amId	assignedId	sdocId	userId	editorUserId	indexActionMentionId	external_id	dbActionMentionId	entity1	semantic_class_entity1	modifier_entity1	actionType	semantic_class_actionType	modifier_actionType	protein_domain_entity1	gene_region_entity1	entity2	semantic_class_entity2	modifier_entity2	protein_domain_entity2	gene_region_entity2	topic	statement_context	negative	certainty_level	derived_certainty_level	applied_rule	indexSentenceId	pmid	sentenceText	procset
44403	2	12	6	10	NULL	0	NULL	asd	NULL		asd	NULL				asd	NULL				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_295_4_1027_s_40	12127999	"`Microsomal"` membrane prepared as described from fresh bovine lens epithelia bound progesterone and corticosterone with high affinity ( Kd 75 nM) ( Fig. 2).	bind
1040	3	12	7	10	NULL	0	NULL	testing	NULL		action test	NULL	mod action 			dfgf	NULL			fgdsg	NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_295_4_1027_s_40	12127999	"`Microsomal"` membrane prepared as described from fresh bovine lens epithelia bound progesterone and corticosterone with high affinity ( Kd 75 nM) ( Fig. 2).	bind
57771	1	201	5	NULL	NULL	0	NULL	Amph2	GP		bind			SH3		dynamin	GP				NULL		0	NULL	NULL	NULL	gw60_embo_17_18_5273_s_218	9736607	( A) Amph2 SH3 and Amph2-SH3deltaDAPS domains bind equally well to dynamin.	bind
57772	2	201	5	NULL	NULL	0	NULL	Amph2	GP		bind			SH3deltaDAPS		dynamin	GP				NULL		0	NULL	NULL	NULL	gw60_embo_17_18_5273_s_218	9736607	( A) Amph2 SH3 and Amph2-SH3deltaDAPS domains bind equally well to dynamin.	bind
1108	1	201	6	NULL	NULL	0	NULL	Amph2	GP		bind			SH3 domain		dynamin	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_18_5273_s_218	9736607	( A) Amph2 SH3 and Amph2-SH3deltaDAPS domains bind equally well to dynamin.	bind
1109	2	201	6	NULL	NULL	0	NULL	Amph2	GP		bind			SH3deltaDAPS		dynamin	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_18_5273_s_218	9736607	( A) Amph2 SH3 and Amph2-SH3deltaDAPS domains bind equally well to dynamin.	bind
57773	1	212	5	NULL	NULL	0	NULL	Bcl-2	GP	deletion mutant	retains			1-82		Bax	GP	binding activity of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_20_11962_s_8	7744846	( A) and an NH -terminal deletion mutant  Bcl-2( 1-82) retained Bax binding activity  in vitro  but failed to suppress Bax-mediated cytotoxicity in yeast.	bind
57774	2	212	5	NULL	NULL	0	NULL	Bax	GP		mediates					cytotoxicity	Process				NULL	yeast	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_20_11962_s_8	7744846	( A) and an NH -terminal deletion mutant  Bcl-2( 1-82) retained Bax binding activity  in vitro  but failed to suppress Bax-mediated cytotoxicity in yeast.	bind
57775	3	212	5	NULL	NULL	0	NULL	Bcl-2	GP	deletion mutant	does not suppress			1-82		statement 2	Process				NULL	yeast	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_20_11962_s_8	7744846	( A) and an NH -terminal deletion mutant  Bcl-2( 1-82) retained Bax binding activity  in vitro  but failed to suppress Bax-mediated cytotoxicity in yeast.	bind
1110	1	212	6	NULL	NULL	0	NULL	Bcl-2	GP		bind			NH -terminal deletion mutant		Bax	GP				NULL	In vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_20_11962_s_8	7744846	( A) and an NH -terminal deletion mutant  Bcl-2( 1-82) retained Bax binding activity  in vitro  but failed to suppress Bax-mediated cytotoxicity in yeast.	bind
1111	3	212	6	NULL	NULL	0	NULL	Bcl-2	GP		does not supress			NH -terminal deletion mutant		Statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_20_11962_s_8	7744846	( A) and an NH -terminal deletion mutant  Bcl-2( 1-82) retained Bax binding activity  in vitro  but failed to suppress Bax-mediated cytotoxicity in yeast.	bind
1112	2	212	6	NULL	NULL	0	NULL	Bax	GP		mediates					cytotoxicity	Process				NULL	yeast	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_20_11962_s_8	7744846	( A) and an NH -terminal deletion mutant  Bcl-2( 1-82) retained Bax binding activity  in vitro  but failed to suppress Bax-mediated cytotoxicity in yeast.	bind
57776	1	218	5	NULL	NULL	0	NULL	cephalexin	GP		bind					BcII	GP	WT			NULL		0	NULL	NULL	NULL	gw70_pnas_102_39_13761_s_140	16172409	( A) and cephalexin ( B) binding to WT BcII (filled circles) and M5 (open circles).	bind
57777	2	218	5	NULL	NULL	0	NULL	cephalexin	GP		bind					M5	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_102_39_13761_s_140	16172409	( A) and cephalexin ( B) binding to WT BcII (filled circles) and M5 (open circles).	bind
1113	1	218	6	NULL	NULL	0	NULL	cephalexin	Chemical		bind					BcII	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_39_13761_s_140	16172409	( A) and cephalexin ( B) binding to WT BcII (filled circles) and M5 (open circles).	bind
1114	2	218	6	NULL	NULL	0	NULL	cephalexin	Chemical		bind					M5	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_39_13761_s_140	16172409	( A) and cephalexin ( B) binding to WT BcII (filled circles) and M5 (open circles).	bind
57778	1	219	5	NULL	NULL	0	NULL	V2R-pp	GP		bind					beta-arrestin 2	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_53_55744_s_141	15501822	( A) and competitive binding of V2R-pp and V2R-np to beta-arrestin 2 ( B).	bind
57779	2	219	5	NULL	NULL	0	NULL	V2R-np	GP		bind					beta-arrestin 2	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_53_55744_s_141	15501822	( A) and competitive binding of V2R-pp and V2R-np to beta-arrestin 2 ( B).	bind
57780	3	219	5	NULL	NULL	0	NULL	statement 1	Process		competes with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_53_55744_s_141	15501822	( A) and competitive binding of V2R-pp and V2R-np to beta-arrestin 2 ( B).	bind
1115	1	219	6	NULL	NULL	0	NULL	V2R-pp	GP		bind					beta-arrestin 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_53_55744_s_141	15501822	( A) and competitive binding of V2R-pp and V2R-np to beta-arrestin 2 ( B).	bind
1116	2	219	6	NULL	NULL	0	NULL	V2R-np	GP		bind					beta-arrestin 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_53_55744_s_141	15501822	( A) and competitive binding of V2R-pp and V2R-np to beta-arrestin 2 ( B).	bind
51765	3	219	6	NULL	NULL	0	NULL	statement 1	process		compete with					statement 2	process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_53_55744_s_141	15501822	( A) and competitive binding of V2R-pp and V2R-np to beta-arrestin 2 ( B).	bind
57781	1	233	5	NULL	NULL	0	NULL	platelets	Cell		is stimulated by					thrombin	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_12_7004_s_178	8636130	( A) and irreversible ( B) binding of PAC-1  to thrombin-stimulated platelets.	bind
57782	2	233	5	NULL	NULL	0	NULL	PAC-1	GP		bind		irreversibly			statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_12_7004_s_178	8636130	( A) and irreversible ( B) binding of PAC-1  to thrombin-stimulated platelets.	bind
1117	2	233	6	NULL	NULL	0	NULL	PAC-1	GP		bind		irreverrsible			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_12_7004_s_178	8636130	( A) and irreversible ( B) binding of PAC-1  to thrombin-stimulated platelets.	bind
51766	1	233	6	NULL	NULL	0	NULL	thrombin	GP		stimulate					platelets	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_12_7004_s_178	8636130	( A) and irreversible ( B) binding of PAC-1  to thrombin-stimulated platelets.	bind
57840	1	235	5	NULL	NULL	0	NULL	mAb	GP		bind					TPO	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_50_35313_s_146	10585396	( A) and mAb 47 binding to untreated TPO and TPO treated by CaCl2 (8 x 10 6M) with or without EDTA (1.6 x 10 4M) ( B).	bind
57841	2	235	5	NULL	NULL	0	NULL	TPO	GP		treated with					CaCl2	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_50_35313_s_146	10585396	( A) and mAb 47 binding to untreated TPO and TPO treated by CaCl2 (8 x 10 6M) with or without EDTA (1.6 x 10 4M) ( B).	bind
57842	3	235	5	NULL	NULL	0	NULL	mAb	GP		bind					statement 1	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_50_35313_s_146	10585396	( A) and mAb 47 binding to untreated TPO and TPO treated by CaCl2 (8 x 10 6M) with or without EDTA (1.6 x 10 4M) ( B).	bind
1118	1	235	6	NULL	NULL	0	NULL	mAb 47	AminoAcid		bind					TPO	GP	untreated			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_50_35313_s_146	10585396	( A) and mAb 47 binding to untreated TPO and TPO treated by CaCl2 (8 x 10 6M) with or without EDTA (1.6 x 10 4M) ( B).	bind
1119	2	235	6	NULL	NULL	0	NULL	mAb 47	AminoAcid		bind					TPO 	GP	CaCl2 treated 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_50_35313_s_146	10585396	( A) and mAb 47 binding to untreated TPO and TPO treated by CaCl2 (8 x 10 6M) with or without EDTA (1.6 x 10 4M) ( B).	bind
57783	1	237	5	NULL	NULL	0	NULL	FV	GP		bind					PS	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_49_51466_s_103	15452129	( A) and MMRN1 did not significantly inhibit FV binding to PS ( B).	bind
57784	2	237	5	NULL	NULL	0	NULL	MMRN1	GP		does not inhibit		significantly			statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_49_51466_s_103	15452129	( A) and MMRN1 did not significantly inhibit FV binding to PS ( B).	bind
1122	1	237	6	NULL	NULL	0	NULL	FV	GP		bind					PS	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_49_51466_s_103	15452129	( A) and MMRN1 did not significantly inhibit FV binding to PS ( B).	bind
1123	2	237	6	NULL	NULL	0	NULL	MMRN1	GP		does not inhibit		significantly 			Statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_49_51466_s_103	15452129	( A) and MMRN1 did not significantly inhibit FV binding to PS ( B).	bind
57794	1	243	5	NULL	NULL	0	NULL	protein phosphatase 1	GP		bind					Yotiao	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_36_31347_s_28	16002409	( A) and protein phosphatase 1 ( 1) are shown bound to Yotiao.	bind
1124	1	243	6	NULL	NULL	0	NULL	protein phosphatase 1	GP		bind					Yotiao	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_31347_s_28	16002409	( A) and protein phosphatase 1 ( 1) are shown bound to Yotiao.	bind
57795	1	248	5	10	NULL	0	NULL	SLV	CellComponent		contains					PS	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_16_11013_s_212	10196183	( A) and TGase 1 bound to SLV containing 15% PS ( B).	bind
57796	2	248	5	NULL	NULL	0	NULL	TGase 1	GP		bind					statement 1	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_16_11013_s_212	10196183	( A) and TGase 1 bound to SLV containing 15% PS ( B).	bind
1125	1	248	6	NULL	NULL	0	NULL	TGase 1	GP		bind					SLV	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_16_11013_s_212	10196183	( A) and TGase 1 bound to SLV containing 15% PS ( B).	bind
57797	1	258	5	NULL	NULL	0	NULL	AP4	GP		bind					PAHX-AP1	GP			PRE	NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_35_13074_s_36	16924111	( A) AP4 binds to the PAHX-AP1 PRE, but Gem does not.	bind
57798	2	258	5	NULL	NULL	0	NULL	Gem	GP		does not bind					PAHX-AP1	GP			PRE	NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_35_13074_s_36	16924111	( A) AP4 binds to the PAHX-AP1 PRE, but Gem does not.	bind
1126	1	258	6	NULL	NULL	0	NULL	AP4	GP		bind					PAHX-AP1	GP			PRE	NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_35_13074_s_36	16924111	( A) AP4 binds to the PAHX-AP1 PRE, but Gem does not.	bind
1127	2	258	6	NULL	NULL	0	NULL	Gem	GP		does not bind					PAHX-AP1	GP			PRE	NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_35_13074_s_36	16924111	( A) AP4 binds to the PAHX-AP1 PRE, but Gem does not.	bind
57799	1	260	5	NULL	NULL	0	NULL	Arp2/3	GP		bind					VCA domain	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_science_290_5492_801_s_73	11052943	( A) Arp2/3  binding to the VCA domain is not blocked by the GBD (residues 196-274)  or control region (178-274).	bind
57800	2	260	5	NULL	NULL	0	NULL		AminoAcid		does not block			GBD (residues 196-274)		statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_science_290_5492_801_s_73	11052943	( A) Arp2/3  binding to the VCA domain is not blocked by the GBD (residues 196-274)  or control region (178-274).	bind
57801	3	260	5	NULL	NULL	0	NULL		AminoAcid		does not block			control region (178-274)		statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_science_290_5492_801_s_73	11052943	( A) Arp2/3  binding to the VCA domain is not blocked by the GBD (residues 196-274)  or control region (178-274).	bind
1128	1	260	6	NULL	NULL	0	NULL	Arp2/3	GP		bind						AminoAcid		VCA domain		NULL		NULL	NULL	NULL	NULL	gw60_science_290_5492_801_s_73	11052943	( A) Arp2/3  binding to the VCA domain is not blocked by the GBD (residues 196-274)  or control region (178-274).	bind
1129	2	260	6	NULL	NULL	0	NULL		AminoAcid		does not block			GBD (residues 196-274)		Statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_290_5492_801_s_73	11052943	( A) Arp2/3  binding to the VCA domain is not blocked by the GBD (residues 196-274)  or control region (178-274).	bind
1130	3	260	6	NULL	NULL	0	NULL		AminoAcid		does not block			control region (178-274)		Statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_290_5492_801_s_73	11052943	( A) Arp2/3  binding to the VCA domain is not blocked by the GBD (residues 196-274)  or control region (178-274).	bind
57802	1	261	5	NULL	NULL	0	NULL	Noxa m3	GP		bind					Mcl-1	GP				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1294_s_196	15901672	( A) As Noxa m3 binds Mcl-1, Bcl-xL, and Bcl-w but not Bcl-2, targeting of these prosurvival proteins suffices for Bak-mediated  apoptosis, whereas neutralization of Bcl-2 is not required.	bind
57803	2	261	5	NULL	NULL	0	NULL	Noxa m3	GP		bind					Bcl-xL	GP				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1294_s_196	15901672	( A) As Noxa m3 binds Mcl-1, Bcl-xL, and Bcl-w but not Bcl-2, targeting of these prosurvival proteins suffices for Bak-mediated  apoptosis, whereas neutralization of Bcl-2 is not required.	bind
57804	3	261	5	NULL	NULL	0	NULL	Noxa m3	GP		bind					Bcl-w	GP				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1294_s_196	15901672	( A) As Noxa m3 binds Mcl-1, Bcl-xL, and Bcl-w but not Bcl-2, targeting of these prosurvival proteins suffices for Bak-mediated  apoptosis, whereas neutralization of Bcl-2 is not required.	bind
57805	4	261	5	NULL	NULL	0	NULL	Noxa m3	GP		does not bind					Bcl-2	GP				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1294_s_196	15901672	( A) As Noxa m3 binds Mcl-1, Bcl-xL, and Bcl-w but not Bcl-2, targeting of these prosurvival proteins suffices for Bak-mediated  apoptosis, whereas neutralization of Bcl-2 is not required.	bind
57806	5	261	5	NULL	NULL	0	NULL	Bak	GP		mediates					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1294_s_196	15901672	( A) As Noxa m3 binds Mcl-1, Bcl-xL, and Bcl-w but not Bcl-2, targeting of these prosurvival proteins suffices for Bak-mediated  apoptosis, whereas neutralization of Bcl-2 is not required.	bind
57807	6	261	5	NULL	NULL	0	NULL	Mcl-1	GP		is a type of					prosurvival protein	GP				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1294_s_196	15901672	( A) As Noxa m3 binds Mcl-1, Bcl-xL, and Bcl-w but not Bcl-2, targeting of these prosurvival proteins suffices for Bak-mediated  apoptosis, whereas neutralization of Bcl-2 is not required.	bind
57808	7	261	5	NULL	NULL	0	NULL	Bcl-xL	GP		is a type of					prosurvival protein	GP				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1294_s_196	15901672	( A) As Noxa m3 binds Mcl-1, Bcl-xL, and Bcl-w but not Bcl-2, targeting of these prosurvival proteins suffices for Bak-mediated  apoptosis, whereas neutralization of Bcl-2 is not required.	bind
57809	8	261	5	NULL	NULL	0	NULL	Bcl-w	GP		is a type of					prosurvival protein	GP				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1294_s_196	15901672	( A) As Noxa m3 binds Mcl-1, Bcl-xL, and Bcl-w but not Bcl-2, targeting of these prosurvival proteins suffices for Bak-mediated  apoptosis, whereas neutralization of Bcl-2 is not required.	bind
57810	9	261	5	NULL	NULL	0	NULL	Bcl-2	GP		is a type of					prosurvival protein	GP				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1294_s_196	15901672	( A) As Noxa m3 binds Mcl-1, Bcl-xL, and Bcl-w but not Bcl-2, targeting of these prosurvival proteins suffices for Bak-mediated  apoptosis, whereas neutralization of Bcl-2 is not required.	bind
57811	10	261	5	NULL	NULL	0	NULL	Mcl-1	GP	targeting of	suffices for					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1294_s_196	15901672	( A) As Noxa m3 binds Mcl-1, Bcl-xL, and Bcl-w but not Bcl-2, targeting of these prosurvival proteins suffices for Bak-mediated  apoptosis, whereas neutralization of Bcl-2 is not required.	bind
57812	11	261	5	NULL	NULL	0	NULL	Bcl-xL	GP		suffices for					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1294_s_196	15901672	( A) As Noxa m3 binds Mcl-1, Bcl-xL, and Bcl-w but not Bcl-2, targeting of these prosurvival proteins suffices for Bak-mediated  apoptosis, whereas neutralization of Bcl-2 is not required.	bind
57813	12	261	5	NULL	NULL	0	NULL	Bcl-w	GP		suffices for					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1294_s_196	15901672	( A) As Noxa m3 binds Mcl-1, Bcl-xL, and Bcl-w but not Bcl-2, targeting of these prosurvival proteins suffices for Bak-mediated  apoptosis, whereas neutralization of Bcl-2 is not required.	bind
1131	1	261	6	NULL	NULL	0	NULL	Noxa m3	GP		bind					Mcl-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_11_1294_s_196	15901672	( A) As Noxa m3 binds Mcl-1, Bcl-xL, and Bcl-w but not Bcl-2, targeting of these prosurvival proteins suffices for Bak-mediated  apoptosis, whereas neutralization of Bcl-2 is not required.	bind
1132	2	261	6	NULL	NULL	0	NULL	Noxa m3	GP		bind					Bcl-xL	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_11_1294_s_196	15901672	( A) As Noxa m3 binds Mcl-1, Bcl-xL, and Bcl-w but not Bcl-2, targeting of these prosurvival proteins suffices for Bak-mediated  apoptosis, whereas neutralization of Bcl-2 is not required.	bind
1133	3	261	6	NULL	NULL	0	NULL	Noxa m3	GP		bind					Bcl-w	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_11_1294_s_196	15901672	( A) As Noxa m3 binds Mcl-1, Bcl-xL, and Bcl-w but not Bcl-2, targeting of these prosurvival proteins suffices for Bak-mediated  apoptosis, whereas neutralization of Bcl-2 is not required.	bind
1134	4	261	6	NULL	NULL	0	NULL	Noxa m3	GP		does not bind					Bcl-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_11_1294_s_196	15901672	( A) As Noxa m3 binds Mcl-1, Bcl-xL, and Bcl-w but not Bcl-2, targeting of these prosurvival proteins suffices for Bak-mediated  apoptosis, whereas neutralization of Bcl-2 is not required.	bind
1135	5	261	6	NULL	NULL	0	NULL	Bak	GP		mediates					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_11_1294_s_196	15901672	( A) As Noxa m3 binds Mcl-1, Bcl-xL, and Bcl-w but not Bcl-2, targeting of these prosurvival proteins suffices for Bak-mediated  apoptosis, whereas neutralization of Bcl-2 is not required.	bind
57814	1	262	5	NULL	NULL	0	NULL	SeqA	GP		bind					GATC sequences within oriC	NucleicAcid	newly generated;;hemimethylated			NULL		NULL	NULL	NULL	NULL	gw70_embo_24_8_1502_s_235	15933720	( A) As replication initiates, SeqA binds newly generated hemimethylated GATC sequences  within  oriC, triggering origin sequestration.	bind
57815	2	262	5	NULL	NULL	0	NULL	statement 1	Process		triggers					origin sequestration	Process				NULL		0	NULL	NULL	NULL	gw70_embo_24_8_1502_s_235	15933720	( A) As replication initiates, SeqA binds newly generated hemimethylated GATC sequences  within  oriC, triggering origin sequestration.	bind
1136	1	262	6	NULL	NULL	0	NULL	SeqA	NucleicAcid		bind					oriC	NucleicAcid	newly generated;;hemimethylated		GATC 	NULL		NULL	NULL	NULL	NULL	gw70_embo_24_8_1502_s_235	15933720	( A) As replication initiates, SeqA binds newly generated hemimethylated GATC sequences  within  oriC, triggering origin sequestration.	bind
1137	2	262	6	NULL	NULL	0	NULL	Statement 1	Process		triggers					origin 	NucleicAcid	sequestration of			NULL		NULL	NULL	NULL	NULL	gw70_embo_24_8_1502_s_235	15933720	( A) As replication initiates, SeqA binds newly generated hemimethylated GATC sequences  within  oriC, triggering origin sequestration.	bind
51767	3	262	6	NULL	NULL	0	NULL	statement 1	Process		occurs after					replication	Process	initiation of			NULL		NULL	NULL	NULL	NULL	gw70_embo_24_8_1502_s_235	15933720	( A) As replication initiates, SeqA binds newly generated hemimethylated GATC sequences  within  oriC, triggering origin sequestration.	bind
57843	1	262	7	NULL	NULL	0	NULL	GATC sequences	GP	hemimethylated	present within					oriC	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_8_1502_s_235	15933720	( A) As replication initiates, SeqA binds newly generated hemimethylated GATC sequences  within  oriC, triggering origin sequestration.	bind
57844	2	262	7	NULL	NULL	0	NULL	SeqA	GP		bind					statement 1	GP	newly generated			NULL		0	NULL	NULL	NULL	gw70_embo_24_8_1502_s_235	15933720	( A) As replication initiates, SeqA binds newly generated hemimethylated GATC sequences  within  oriC, triggering origin sequestration.	bind
57845	3	262	7	NULL	NULL	0	NULL	statement 2	Process		occur during					replication	Process	initiation of			NULL		0	NULL	NULL	NULL	gw70_embo_24_8_1502_s_235	15933720	( A) As replication initiates, SeqA binds newly generated hemimethylated GATC sequences  within  oriC, triggering origin sequestration.	bind
57846	4	262	7	NULL	NULL	0	NULL	statement 2	Process		trigger					origin sequestration	Process				NULL		0	NULL	NULL	NULL	gw70_embo_24_8_1502_s_235	15933720	( A) As replication initiates, SeqA binds newly generated hemimethylated GATC sequences  within  oriC, triggering origin sequestration.	bind
57816	1	349	5	NULL	NULL	0	NULL	SRC1	GP		bind					FXR	GP				NULL		0	NULL	NULL	NULL	gw60_science_284_5418_1365_s_63	10334993	( A) CDCA and its conjugates increase SRC1 binding to FXR.	bind
57817	2	349	5	NULL	NULL	0	NULL	CDCA	GP		increases					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_science_284_5418_1365_s_63	10334993	( A) CDCA and its conjugates increase SRC1 binding to FXR.	bind
1138	1	349	6	NULL	NULL	0	NULL	SRC1	GP		bind					FXR	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5418_1365_s_63	10334993	( A) CDCA and its conjugates increase SRC1 binding to FXR.	bind
1139	2	349	6	NULL	NULL	0	NULL	CDCA	Chemical		increase					Statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5418_1365_s_63	10334993	( A) CDCA and its conjugates increase SRC1 binding to FXR.	bind
57818	1	351	5	NULL	NULL	0	NULL	CED-4	GP		bind					CED-9	GP				NULL		0	NULL	NULL	NULL	gw60_science_275_5303_1122_s_90	9027312	( A) CED-4 binds CED-9.	bind
1140	1	351	6	NULL	NULL	0	NULL	CED-4	GP		bind					CED-9	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_275_5303_1122_s_90	9027312	( A) CED-4 binds CED-9.	bind
57819	1	354	5	NULL	NULL	0	NULL	Cellular proteins	GP		is associated with					Grb2	GP				NULL		0	NULL	NULL	NULL	gw60_embo_20_22_6337_s_167	11707405	( A) Cellular proteins associated with Grb2 bound to MT mutants.	bind
57820	2	354	5	NULL	NULL	0	NULL	statement 1	GP		bind					MT	GP	mutant			NULL		0	NULL	NULL	NULL	gw60_embo_20_22_6337_s_167	11707405	( A) Cellular proteins associated with Grb2 bound to MT mutants.	bind
1141	1	354	6	NULL	NULL	0	NULL	Grb2	GP		bind					MT	CellComponent	mutant			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_22_6337_s_167	11707405	( A) Cellular proteins associated with Grb2 bound to MT mutants.	bind
51768	2	354	6	NULL	NULL	0	NULL	Cellular proteins	GP		associate with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_22_6337_s_167	11707405	( A) Cellular proteins associated with Grb2 bound to MT mutants.	bind
1207	1	370	6	NULL	NULL	0	NULL	dopamine	Chemical		compete with					E-HRP	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_155	11027358	( A) Competition of E-HRP binding by the catecholamines dopamine (Dpn), NE, and epinephrine (E) and the catecholestrogen 2-hydroxyestradiol.	bind
1208	2	370	6	NULL	NULL	0	NULL	NE	Chemical		compete with					E-HRP	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_155	11027358	( A) Competition of E-HRP binding by the catecholamines dopamine (Dpn), NE, and epinephrine (E) and the catecholestrogen 2-hydroxyestradiol.	bind
1209	3	370	6	NULL	NULL	0	NULL	epinephrine	Chemical		compete with					E-HRP	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_155	11027358	( A) Competition of E-HRP binding by the catecholamines dopamine (Dpn), NE, and epinephrine (E) and the catecholestrogen 2-hydroxyestradiol.	bind
1210	4	370	6	NULL	NULL	0	NULL	2-hydroxyestradiol	Chemical		compete with					E-HRP	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_155	11027358	( A) Competition of E-HRP binding by the catecholamines dopamine (Dpn), NE, and epinephrine (E) and the catecholestrogen 2-hydroxyestradiol.	bind
51769	5	370	6	NULL	NULL	0	NULL	Dpn	Chemical		is					dopamine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_155	11027358	( A) Competition of E-HRP binding by the catecholamines dopamine (Dpn), NE, and epinephrine (E) and the catecholestrogen 2-hydroxyestradiol.	bind
51770	6	370	6	NULL	NULL	0	NULL	E	Chemical		is 					epinephrine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_155	11027358	( A) Competition of E-HRP binding by the catecholamines dopamine (Dpn), NE, and epinephrine (E) and the catecholestrogen 2-hydroxyestradiol.	bind
51771	7	370	6	NULL	NULL	0	NULL	dopamine	Chemical		is a type of					catecholamine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_155	11027358	( A) Competition of E-HRP binding by the catecholamines dopamine (Dpn), NE, and epinephrine (E) and the catecholestrogen 2-hydroxyestradiol.	bind
51772	8	370	6	NULL	NULL	0	NULL	NE	Chemical		is a type of					catecholamine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_155	11027358	( A) Competition of E-HRP binding by the catecholamines dopamine (Dpn), NE, and epinephrine (E) and the catecholestrogen 2-hydroxyestradiol.	bind
51773	9	370	6	NULL	NULL	0	NULL	E	Chemical		is a type of					catecholamine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_155	11027358	( A) Competition of E-HRP binding by the catecholamines dopamine (Dpn), NE, and epinephrine (E) and the catecholestrogen 2-hydroxyestradiol.	bind
51774	10	370	6	NULL	NULL	0	NULL	2-hydroxyestradiol	Chemical		is a type of					catecholestrogen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_155	11027358	( A) Competition of E-HRP binding by the catecholamines dopamine (Dpn), NE, and epinephrine (E) and the catecholestrogen 2-hydroxyestradiol.	bind
57821	1	371	5	NULL	NULL	0	NULL	hnRNP A1	GP	endogenous	bind					MHV RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_17_4701_s_177	10970862	( A) Competition of the binding of endogenous hnRNP A1 to MHV RNA by hnRNP A1deltaC.	bind
57822	2	371	5	NULL	NULL	0	NULL	hnRNP A1deltaC	GP		bind					MHV RNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4701_s_177	10970862	( A) Competition of the binding of endogenous hnRNP A1 to MHV RNA by hnRNP A1deltaC.	bind
57823	3	371	5	NULL	NULL	0	NULL	statement 2	Process		competes with					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4701_s_177	10970862	( A) Competition of the binding of endogenous hnRNP A1 to MHV RNA by hnRNP A1deltaC.	bind
1211	1	371	6	NULL	NULL	0	NULL	hnRNP A1	GP	endogenous	bind					MHV RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_17_4701_s_177	10970862	( A) Competition of the binding of endogenous hnRNP A1 to MHV RNA by hnRNP A1deltaC.	bind
1212	2	371	6	NULL	NULL	0	NULL	hnRNP A1deltaC	GP		bind					MHV RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_17_4701_s_177	10970862	( A) Competition of the binding of endogenous hnRNP A1 to MHV RNA by hnRNP A1deltaC.	bind
51775	3	371	6	NULL	NULL	0	NULL	statement 1	Process		compete with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_17_4701_s_177	10970862	( A) Competition of the binding of endogenous hnRNP A1 to MHV RNA by hnRNP A1deltaC.	bind
57824	1	377	5	NULL	NULL	0	NULL	E1	GP		bind		cooperatively	DBD		E2	GP		DBD		NULL		0	NULL	NULL	NULL	gw60_embo_19_12_3069_s_187	10856250	( A) Cooperative binding of E1 and E2 DBDs is disrupted by a double point mutation between the two sites.	bind
1213	1	377	6	NULL	NULL	0	NULL	E1	GP		bind		cooperatively	DBD		E2	GP		DBD		NULL		NULL	NULL	NULL	NULL	gw60_embo_19_12_3069_s_187	10856250	( A) Cooperative binding of E1 and E2 DBDs is disrupted by a double point mutation between the two sites.	bind
57825	1	378	5	NULL	NULL	0	NULL	capsids	GP	CPV	bind					TfR	GP	feline			NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_59_0_553_s_287	16153179	( a) CPV and FPV capsids bind to the feline TfR, but only CPV capsids bind the canine  TfR.	bind
57826	2	378	5	NULL	NULL	0	NULL	capsids	GP	FPV	bind					TfR	GP	feline			NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_59_0_553_s_287	16153179	( a) CPV and FPV capsids bind to the feline TfR, but only CPV capsids bind the canine  TfR.	bind
57827	3	378	5	NULL	NULL	0	NULL	capsids	GP	CPV	bind					TfR	GP	canine			NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_59_0_553_s_287	16153179	( a) CPV and FPV capsids bind to the feline TfR, but only CPV capsids bind the canine  TfR.	bind
1215	1	378	6	NULL	NULL	0	NULL	CPV capsid	CellComponent		bind					TfR	GP	feline			NULL		NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_59_0_553_s_287	16153179	( a) CPV and FPV capsids bind to the feline TfR, but only CPV capsids bind the canine  TfR.	bind
1216	2	378	6	NULL	NULL	0	NULL	FPV capsid	CellComponent		bind					TfR	GP	feline			NULL		NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_59_0_553_s_287	16153179	( a) CPV and FPV capsids bind to the feline TfR, but only CPV capsids bind the canine  TfR.	bind
1217	3	378	6	NULL	NULL	0	NULL	CPV capsid	CellComponent		bind					TfR	GP	canine			NULL		NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_59_0_553_s_287	16153179	( a) CPV and FPV capsids bind to the feline TfR, but only CPV capsids bind the canine  TfR.	bind
57828	1	386	5	NULL	NULL	0	NULL	GAPDH	GP		bind					Siah1	GP				NULL	in vitro	0	NULL	NULL	NULL	gw70_pnas_103_10_3887_s_35	16505364	( a) Deprenyl (DEP) inhibits the binding of GAPDH and Siah1  in vitro.	bind
57829	2	386	5	NULL	NULL	0	NULL	DEP	Chemical		is					Deprenyl	Chemical				NULL		0	NULL	NULL	NULL	gw70_pnas_103_10_3887_s_35	16505364	( a) Deprenyl (DEP) inhibits the binding of GAPDH and Siah1  in vitro.	bind
57830	3	386	5	NULL	NULL	0	NULL	DEP	Chemical		inhibits					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_103_10_3887_s_35	16505364	( a) Deprenyl (DEP) inhibits the binding of GAPDH and Siah1  in vitro.	bind
1218	1	386	6	NULL	NULL	0	NULL	GAPDH	GP		bind					Siah1	GP				NULL	In vitro	NULL	NULL	NULL	NULL	gw70_pnas_103_10_3887_s_35	16505364	( a) Deprenyl (DEP) inhibits the binding of GAPDH and Siah1  in vitro.	bind
1219	2	386	6	NULL	NULL	0	NULL	Deprenyl 	Chemical		inhibits					Statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_10_3887_s_35	16505364	( a) Deprenyl (DEP) inhibits the binding of GAPDH and Siah1  in vitro.	bind
51776	3	386	6	NULL	NULL	0	NULL	DEP	Chemical		is					Deprenyl	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_10_3887_s_35	16505364	( a) Deprenyl (DEP) inhibits the binding of GAPDH and Siah1  in vitro.	bind
57831	1	387	5	NULL	NULL	0	NULL	IDH2	GP		bind			catalytic site		isocitrate	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_15_12864_s_267	12562755	( A) Despite residue differences in the isocitrate binding sites, the catalytic site in IDH2 and the regulatory site in IDH1 bind isocitrate with similar affinity.	bind
57832	2	387	5	NULL	NULL	0	NULL	IDH1	GP		bind			regulatory site		isocitrate	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_15_12864_s_267	12562755	( A) Despite residue differences in the isocitrate binding sites, the catalytic site in IDH2 and the regulatory site in IDH1 bind isocitrate with similar affinity.	bind
57833	3	387	5	NULL	NULL	0	NULL	statement 1	Process	affinity of	is similar to					statement 2	Process	affinity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_15_12864_s_267	12562755	( A) Despite residue differences in the isocitrate binding sites, the catalytic site in IDH2 and the regulatory site in IDH1 bind isocitrate with similar affinity.	bind
1220	1	387	6	NULL	NULL	0	NULL	IDH2	GP		bind			catalytic site		isocitrate	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_15_12864_s_267	12562755	( A) Despite residue differences in the isocitrate binding sites, the catalytic site in IDH2 and the regulatory site in IDH1 bind isocitrate with similar affinity.	bind
1221	2	387	6	NULL	NULL	0	NULL	IDH1	GP		bind			regulatory site		isocitrate	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_15_12864_s_267	12562755	( A) Despite residue differences in the isocitrate binding sites, the catalytic site in IDH2 and the regulatory site in IDH1 bind isocitrate with similar affinity.	bind
51777	3	387	6	NULL	NULL	0	NULL	statement 1	Process	affinity of	is similar to					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_15_12864_s_267	12562755	( A) Despite residue differences in the isocitrate binding sites, the catalytic site in IDH2 and the regulatory site in IDH1 bind isocitrate with similar affinity.	bind
57834	1	391	5	NULL	NULL	0	NULL	Dsk2p	GP		bind		directly			tetra-Ub	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_2_745_s_133	11805328	( A) Direct binding of Dsk2p to tetra-Ub.	bind
1222	1	391	6	NULL	NULL	0	NULL	Dsk2p	GP		bind		directly			tetra-Ub	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_2_745_s_133	11805328	( A) Direct binding of Dsk2p to tetra-Ub.	bind
57835	1	392	5	NULL	NULL	0	NULL	Hsps	GP		bind					Tdag51	GP				NULL		0	NULL	NULL	NULL	gw70_embo_25_20_4773_s_112	17024176	( A) Direct binding of Hsps with Tdag51.	bind
1223	1	392	6	NULL	NULL	0	NULL	Hsps	GP		bind		directly			Tdag51	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_20_4773_s_112	17024176	( A) Direct binding of Hsps with Tdag51.	bind
57836	1	393	5	NULL	NULL	0	NULL	TLP	GP		bind					TFIIA	GP				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_8_2127_s_168	12682363	( A) Direct binding of TLP and TFIIA.	bind
1224	1	393	6	NULL	NULL	0	NULL	TLP	GP		bind		directly			TFIIA	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_8_2127_s_168	12682363	( A) Direct binding of TLP and TFIIA.	bind
57837	1	398	5	NULL	NULL	0	NULL	NCI-65828	Chemical		docks					AccD5	GP		acyl-CoA-binding pocket		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_9_3072_s_149	16492739	( A) Docking of NCI-65828 in the acyl-CoA-binding pocket of AccD5 matches the binding  motif of an acyl-CoA, in which the anionic sulfate of NCI-65828 binds the entrance  of the CoA pocket and the hydrophobic moiety binds the hydrophobic interior of the  CoA pocket.	bind
57838	2	398	5	NULL	NULL	0	NULL	NCI-65828	Chemical	anionic sulfate of	bind					CoA pocket	AminoAcid	entrance of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_9_3072_s_149	16492739	( A) Docking of NCI-65828 in the acyl-CoA-binding pocket of AccD5 matches the binding  motif of an acyl-CoA, in which the anionic sulfate of NCI-65828 binds the entrance  of the CoA pocket and the hydrophobic moiety binds the hydrophobic interior of the  CoA pocket.	bind
57839	3	398	5	NULL	NULL	0	NULL	NCI-65828	Chemical	hydrophobic moiety of	bind					CoA pocket	AminoAcid	hydrophobic interior of			NULL		0	NULL	NULL	NULL	gw70_pnas_103_9_3072_s_149	16492739	( A) Docking of NCI-65828 in the acyl-CoA-binding pocket of AccD5 matches the binding  motif of an acyl-CoA, in which the anionic sulfate of NCI-65828 binds the entrance  of the CoA pocket and the hydrophobic moiety binds the hydrophobic interior of the  CoA pocket.	bind
1225	1	398	6	NULL	NULL	0	NULL	NCI-65828 	Chemical		bind			anionic sulfate		AccD5	GP		entrance of the CoA pocket		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_9_3072_s_149	16492739	( A) Docking of NCI-65828 in the acyl-CoA-binding pocket of AccD5 matches the binding  motif of an acyl-CoA, in which the anionic sulfate of NCI-65828 binds the entrance  of the CoA pocket and the hydrophobic moiety binds the hydrophobic interior of the  CoA pocket.	bind
1226	2	398	6	NULL	NULL	0	NULL	NCI-65828 	Chemical		bind			hydrophobic moiety		AccD5	GP		hydrophobic interior of the CoA pocket		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_9_3072_s_149	16492739	( A) Docking of NCI-65828 in the acyl-CoA-binding pocket of AccD5 matches the binding  motif of an acyl-CoA, in which the anionic sulfate of NCI-65828 binds the entrance  of the CoA pocket and the hydrophobic moiety binds the hydrophobic interior of the  CoA pocket.	bind
57920	1	401	5	NULL	NULL	0	NULL	anti-CD81	GP		bind					B cells	Cell				NULL		0	NULL	NULL	NULL	gw60_science_282_5390_938_s_43	9794763	( A) Dose-dependent inhibition of anti-CD81 binding to B cells by recombinant E2.	bind
57921	2	401	5	NULL	NULL	0	NULL	E2	GP	recombinant	inhibits		dose dependently			statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_science_282_5390_938_s_43	9794763	( A) Dose-dependent inhibition of anti-CD81 binding to B cells by recombinant E2.	bind
1227	1	401	6	NULL	NULL	0	NULL	anti-CD81	GP		bind					B cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_science_282_5390_938_s_43	9794763	( A) Dose-dependent inhibition of anti-CD81 binding to B cells by recombinant E2.	bind
1228	2	401	6	NULL	NULL	0	NULL	E2	GP	recombinant	inhibits		dose-dependently			Statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_282_5390_938_s_43	9794763	( A) Dose-dependent inhibition of anti-CD81 binding to B cells by recombinant E2.	bind
57922	1	403	5	NULL	NULL	0	NULL	Notch1	GP	activated	down-modulates					Wnts gene	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_genesdev_19_12_1485_s_64	15964998	( A) Down-modulation of  Wnts gene expression by activated Notch1.	bind
1229	1	403	6	NULL	NULL	0	NULL	Notch1	GP	activated	downregulates					Wnts gene	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_12_1485_s_64	15964998	( A) Down-modulation of  Wnts gene expression by activated Notch1.	bind
57923	1	405	5	NULL	NULL	0	NULL	dsDNA	NucleicAcid		bind					Cdc6-1 proteins	GP				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_15_4940_s_135	16150924	( A) dsDNA binding of Cdc6-1 proteins; ( B) ssDNA binding of Cdc6-1 proteins; ( C) dsDNA binding of Cdc6-2 proteins; ( D) ssDNA binding of Cdc6-2 proteins.	bind
57924	2	405	5	NULL	NULL	0	NULL	ssDNA	NucleicAcid		bind					Cdc6-1 proteins	GP				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_15_4940_s_135	16150924	( A) dsDNA binding of Cdc6-1 proteins; ( B) ssDNA binding of Cdc6-1 proteins; ( C) dsDNA binding of Cdc6-2 proteins; ( D) ssDNA binding of Cdc6-2 proteins.	bind
57925	3	405	5	NULL	NULL	0	NULL	dsDNA	NucleicAcid		bind					Cdc6-2 proteins	GP				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_15_4940_s_135	16150924	( A) dsDNA binding of Cdc6-1 proteins; ( B) ssDNA binding of Cdc6-1 proteins; ( C) dsDNA binding of Cdc6-2 proteins; ( D) ssDNA binding of Cdc6-2 proteins.	bind
57926	4	405	5	NULL	NULL	0	NULL	ssDNA	NucleicAcid		bind					Cdc6-2 proteins	GP				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_15_4940_s_135	16150924	( A) dsDNA binding of Cdc6-1 proteins; ( B) ssDNA binding of Cdc6-1 proteins; ( C) dsDNA binding of Cdc6-2 proteins; ( D) ssDNA binding of Cdc6-2 proteins.	bind
1230	1	405	6	NULL	NULL	0	NULL	dsDNA	NucleicAcid		bind					Cdc6-1 proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_15_4940_s_135	16150924	( A) dsDNA binding of Cdc6-1 proteins; ( B) ssDNA binding of Cdc6-1 proteins; ( C) dsDNA binding of Cdc6-2 proteins; ( D) ssDNA binding of Cdc6-2 proteins.	bind
1231	2	405	6	NULL	NULL	0	NULL	ssDNA	NucleicAcid		bind					Cdc6-1 proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_15_4940_s_135	16150924	( A) dsDNA binding of Cdc6-1 proteins; ( B) ssDNA binding of Cdc6-1 proteins; ( C) dsDNA binding of Cdc6-2 proteins; ( D) ssDNA binding of Cdc6-2 proteins.	bind
1232	3	405	6	NULL	NULL	0	NULL	dsDNA	NucleicAcid		bind					cdc6-2 proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_15_4940_s_135	16150924	( A) dsDNA binding of Cdc6-1 proteins; ( B) ssDNA binding of Cdc6-1 proteins; ( C) dsDNA binding of Cdc6-2 proteins; ( D) ssDNA binding of Cdc6-2 proteins.	bind
1233	4	405	6	NULL	NULL	0	NULL	ssDNA	NucleicAcid		bind					Cdc6-2 proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_15_4940_s_135	16150924	( A) dsDNA binding of Cdc6-1 proteins; ( B) ssDNA binding of Cdc6-1 proteins; ( C) dsDNA binding of Cdc6-2 proteins; ( D) ssDNA binding of Cdc6-2 proteins.	bind
57927	1	407	5	NULL	NULL	0	NULL	Fos/Jun heterodimers	GP		bind					TNF	GP			TRE site in promoter	NULL		0	NULL	NULL	NULL	gw60_jclininvest_104_4_503_s_210	10449442	( a) E2 decreases the binding of Fos/Jun heterodimers to the TRE site in the TNF promoter.	bind
57928	2	407	5	NULL	NULL	0	NULL	E2	GP		decreases					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jclininvest_104_4_503_s_210	10449442	( a) E2 decreases the binding of Fos/Jun heterodimers to the TRE site in the TNF promoter.	bind
1234	1	407	6	NULL	NULL	0	NULL	Fos/Jun heterodimer	GP		bind					TNF 	GP			TRE site in promoter	NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_104_4_503_s_210	10449442	( a) E2 decreases the binding of Fos/Jun heterodimers to the TRE site in the TNF promoter.	bind
1235	2	407	6	NULL	NULL	0	NULL	E2	GP		decreases 					Statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_104_4_503_s_210	10449442	( a) E2 decreases the binding of Fos/Jun heterodimers to the TRE site in the TNF promoter.	bind
1236	1	408	6	NULL	NULL	0	NULL	E2F-1-ER	GP		bind					BMI1 	GP			Promoter	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_6_1745_s_147	16582100	( A) E2F-1-ER binds to the  BMI1 promoter upon activation by 4-OHT. Crosslinked chromatin was isolated from untreated  and 4-OHT treated 1A3 cells and precipitated with an E2F-1 specific antibody or a  control antibody.	bind
1507	2	408	6	NULL	NULL	0	NULL	4-OHT	Chemical		activates					Statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_6_1745_s_147	16582100	( A) E2F-1-ER binds to the  BMI1 promoter upon activation by 4-OHT. Crosslinked chromatin was isolated from untreated  and 4-OHT treated 1A3 cells and precipitated with an E2F-1 specific antibody or a  control antibody.	bind
1508	4	408	6	NULL	NULL	0	NULL	chromatin	Chromosome	crosslinked	precipates					E2F-1 specific antibody	GP				NULL	untreated 1A3 cells	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_6_1745_s_147	16582100	( A) E2F-1-ER binds to the  BMI1 promoter upon activation by 4-OHT. Crosslinked chromatin was isolated from untreated  and 4-OHT treated 1A3 cells and precipitated with an E2F-1 specific antibody or a  control antibody.	bind
1509	5	408	6	NULL	NULL	0	NULL	chromatin	Chromosome	crosslinked	precipates					E2F-1 specific antibody	GP				NULL	4-OHT treated 1A3 cells	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_6_1745_s_147	16582100	( A) E2F-1-ER binds to the  BMI1 promoter upon activation by 4-OHT. Crosslinked chromatin was isolated from untreated  and 4-OHT treated 1A3 cells and precipitated with an E2F-1 specific antibody or a  control antibody.	bind
57929	1	409	5	NULL	NULL	0	NULL	E2F7	GP		bind					E2F sites	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_embo_22_23_6289_s_118	14633988	( A) E2F7 binds E2F sites.	bind
1237	1	409	6	NULL	NULL	0	NULL	E2F7	GP		bind						GP			E2F site	NULL		NULL	NULL	NULL	NULL	gw70_embo_22_23_6289_s_118	14633988	( A) E2F7 binds E2F sites.	bind
57930	1	410	5	NULL	NULL	0	NULL	Ebp1	GP		bind					Akt	GP				NULL	nuclear extract	0	NULL	NULL	NULL	gw70_embo_25_10_2083_s_132	16642037	( A) Ebp1 binds Akt in the nuclear extract.	bind
1238	1	410	6	NULL	NULL	0	NULL	Ebp1	GP		bind					Akt	GP				NULL	nuclear extract	NULL	NULL	NULL	NULL	gw70_embo_25_10_2083_s_132	16642037	( A) Ebp1 binds Akt in the nuclear extract.	bind
57931	1	411	5	NULL	NULL	0	NULL	rapamycin	Chemical		effects		possibly			eIF2alpha	GP	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_genesdev_17_7_859_s_73	12654728	( A) Effect of rapamycin on phosphorylation of eIF2alpha is strongly dependent on dephosphorylation of Ser 577 and the tRNA binding activity of GCN2.	bind
57932	2	411	5	NULL	NULL	0	NULL	statement 1	Process		is dependent on		strongly			Ser 577	AminoAcid	dephosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_7_859_s_73	12654728	( A) Effect of rapamycin on phosphorylation of eIF2alpha is strongly dependent on dephosphorylation of Ser 577 and the tRNA binding activity of GCN2.	bind
57933	3	411	5	NULL	NULL	0	NULL	GCN2	GP		bind					tRNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_genesdev_17_7_859_s_73	12654728	( A) Effect of rapamycin on phosphorylation of eIF2alpha is strongly dependent on dephosphorylation of Ser 577 and the tRNA binding activity of GCN2.	bind
57934	4	411	5	NULL	NULL	0	NULL	statement 1	Process		is dependent on		strongly			statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_genesdev_17_7_859_s_73	12654728	( A) Effect of rapamycin on phosphorylation of eIF2alpha is strongly dependent on dephosphorylation of Ser 577 and the tRNA binding activity of GCN2.	bind
1503	1	411	6	NULL	NULL	0	NULL	rapamycin	Chemical		effects					eIF2alpha	GP	phosphorylation of 			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_7_859_s_73	12654728	( A) Effect of rapamycin on phosphorylation of eIF2alpha is strongly dependent on dephosphorylation of Ser 577 and the tRNA binding activity of GCN2.	bind
1504	2	411	6	NULL	NULL	0	NULL	GCN2	GP		bind					tRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_7_859_s_73	12654728	( A) Effect of rapamycin on phosphorylation of eIF2alpha is strongly dependent on dephosphorylation of Ser 577 and the tRNA binding activity of GCN2.	bind
1505	3	411	6	NULL	NULL	0	NULL	Statement 1	Relationship		dependent on		strongly			Ser 577	AminoAcid	dephosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_7_859_s_73	12654728	( A) Effect of rapamycin on phosphorylation of eIF2alpha is strongly dependent on dephosphorylation of Ser 577 and the tRNA binding activity of GCN2.	bind
1506	4	411	6	NULL	NULL	0	NULL	Statement 1	Relationship		dependent on		strongly			Statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_7_859_s_73	12654728	( A) Effect of rapamycin on phosphorylation of eIF2alpha is strongly dependent on dephosphorylation of Ser 577 and the tRNA binding activity of GCN2.	bind
1070	1	415	5	NULL	NULL	0	NULL	eIF2B	GP		does not catalyze					GDP	Chemical	exchange of			NULL	on eIF2(alphaP)	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_12841_s_158	9582312	( a) eIF2B reportedly does not catalyze GDP exchange on eIF2(alphaP) ( 15); ( b) eIF2(alphaP) displaces unphosphorylated eIF2 bound to eIF2B but unphosphorylated eIF2 does not ( 16); and ( c) eIF2(alphaP) inhibits the activity of eIF2B in the presence of low concentrations of substrate ( i.e. <10-fold molar excess of eIF2.GDP to eIF2(alphaP)) but at higher substrate concentrations the inhibition caused by eIF2(alphaP) is negligible ( 15), suggesting that eIF2(alphaP) is acting as a competitive inhibitor of eIF2B.	bind
1071	2	415	5	NULL	NULL	0	NULL	eIF2	GP	unphosphorylated	bind					eIF2B	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_12841_s_158	9582312	( a) eIF2B reportedly does not catalyze GDP exchange on eIF2(alphaP) ( 15); ( b) eIF2(alphaP) displaces unphosphorylated eIF2 bound to eIF2B but unphosphorylated eIF2 does not ( 16); and ( c) eIF2(alphaP) inhibits the activity of eIF2B in the presence of low concentrations of substrate ( i.e. <10-fold molar excess of eIF2.GDP to eIF2(alphaP)) but at higher substrate concentrations the inhibition caused by eIF2(alphaP) is negligible ( 15), suggesting that eIF2(alphaP) is acting as a competitive inhibitor of eIF2B.	bind
1072	3	415	5	NULL	NULL	0	NULL	eIF2(alphaP)	GP		displaces					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_12841_s_158	9582312	( a) eIF2B reportedly does not catalyze GDP exchange on eIF2(alphaP) ( 15); ( b) eIF2(alphaP) displaces unphosphorylated eIF2 bound to eIF2B but unphosphorylated eIF2 does not ( 16); and ( c) eIF2(alphaP) inhibits the activity of eIF2B in the presence of low concentrations of substrate ( i.e. <10-fold molar excess of eIF2.GDP to eIF2(alphaP)) but at higher substrate concentrations the inhibition caused by eIF2(alphaP) is negligible ( 15), suggesting that eIF2(alphaP) is acting as a competitive inhibitor of eIF2B.	bind
1073	4	415	5	NULL	NULL	0	NULL	eIF2	GP	unphosphorylated	does not displace					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_12841_s_158	9582312	( a) eIF2B reportedly does not catalyze GDP exchange on eIF2(alphaP) ( 15); ( b) eIF2(alphaP) displaces unphosphorylated eIF2 bound to eIF2B but unphosphorylated eIF2 does not ( 16); and ( c) eIF2(alphaP) inhibits the activity of eIF2B in the presence of low concentrations of substrate ( i.e. <10-fold molar excess of eIF2.GDP to eIF2(alphaP)) but at higher substrate concentrations the inhibition caused by eIF2(alphaP) is negligible ( 15), suggesting that eIF2(alphaP) is acting as a competitive inhibitor of eIF2B.	bind
1074	5	415	5	NULL	NULL	0	NULL	eIF2(alphaP)	GP		inhibit 					eIF2B	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_12841_s_158	9582312	( a) eIF2B reportedly does not catalyze GDP exchange on eIF2(alphaP) ( 15); ( b) eIF2(alphaP) displaces unphosphorylated eIF2 bound to eIF2B but unphosphorylated eIF2 does not ( 16); and ( c) eIF2(alphaP) inhibits the activity of eIF2B in the presence of low concentrations of substrate ( i.e. <10-fold molar excess of eIF2.GDP to eIF2(alphaP)) but at higher substrate concentrations the inhibition caused by eIF2(alphaP) is negligible ( 15), suggesting that eIF2(alphaP) is acting as a competitive inhibitor of eIF2B.	bind
1075	6	415	5	NULL	NULL	0	NULL	eIF2(alphaP)  	GP		inhibit		negligible			eIF2B	GP	activity			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_12841_s_158	9582312	( a) eIF2B reportedly does not catalyze GDP exchange on eIF2(alphaP) ( 15); ( b) eIF2(alphaP) displaces unphosphorylated eIF2 bound to eIF2B but unphosphorylated eIF2 does not ( 16); and ( c) eIF2(alphaP) inhibits the activity of eIF2B in the presence of low concentrations of substrate ( i.e. <10-fold molar excess of eIF2.GDP to eIF2(alphaP)) but at higher substrate concentrations the inhibition caused by eIF2(alphaP) is negligible ( 15), suggesting that eIF2(alphaP) is acting as a competitive inhibitor of eIF2B.	bind
1076	7	415	5	NULL	NULL	0	NULL	eIF2(alphaP)	GP		inhibit		competitively			eIF2B	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_12841_s_158	9582312	( a) eIF2B reportedly does not catalyze GDP exchange on eIF2(alphaP) ( 15); ( b) eIF2(alphaP) displaces unphosphorylated eIF2 bound to eIF2B but unphosphorylated eIF2 does not ( 16); and ( c) eIF2(alphaP) inhibits the activity of eIF2B in the presence of low concentrations of substrate ( i.e. <10-fold molar excess of eIF2.GDP to eIF2(alphaP)) but at higher substrate concentrations the inhibition caused by eIF2(alphaP) is negligible ( 15), suggesting that eIF2(alphaP) is acting as a competitive inhibitor of eIF2B.	bind
52129	8	415	5	NULL	NULL	0	NULL	statement 5	Process		in the presence of					substrate	GP	low concentration of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_12841_s_158	9582312	( a) eIF2B reportedly does not catalyze GDP exchange on eIF2(alphaP) ( 15); ( b) eIF2(alphaP) displaces unphosphorylated eIF2 bound to eIF2B but unphosphorylated eIF2 does not ( 16); and ( c) eIF2(alphaP) inhibits the activity of eIF2B in the presence of low concentrations of substrate ( i.e. <10-fold molar excess of eIF2.GDP to eIF2(alphaP)) but at higher substrate concentrations the inhibition caused by eIF2(alphaP) is negligible ( 15), suggesting that eIF2(alphaP) is acting as a competitive inhibitor of eIF2B.	bind
52130	9	415	5	NULL	NULL	0	NULL	statement 6	Process		in the presence of					substrate	GP	high concentration of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_12841_s_158	9582312	( a) eIF2B reportedly does not catalyze GDP exchange on eIF2(alphaP) ( 15); ( b) eIF2(alphaP) displaces unphosphorylated eIF2 bound to eIF2B but unphosphorylated eIF2 does not ( 16); and ( c) eIF2(alphaP) inhibits the activity of eIF2B in the presence of low concentrations of substrate ( i.e. <10-fold molar excess of eIF2.GDP to eIF2(alphaP)) but at higher substrate concentrations the inhibition caused by eIF2(alphaP) is negligible ( 15), suggesting that eIF2(alphaP) is acting as a competitive inhibitor of eIF2B.	bind
1512	1	415	6	NULL	NULL	0	NULL	eIF2	GP	unphosphorylated	bind					eIF2B	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_12841_s_158	9582312	( a) eIF2B reportedly does not catalyze GDP exchange on eIF2(alphaP) ( 15); ( b) eIF2(alphaP) displaces unphosphorylated eIF2 bound to eIF2B but unphosphorylated eIF2 does not ( 16); and ( c) eIF2(alphaP) inhibits the activity of eIF2B in the presence of low concentrations of substrate ( i.e. <10-fold molar excess of eIF2.GDP to eIF2(alphaP)) but at higher substrate concentrations the inhibition caused by eIF2(alphaP) is negligible ( 15), suggesting that eIF2(alphaP) is acting as a competitive inhibitor of eIF2B.	bind
1513	2	415	6	NULL	NULL	0	NULL	eIF2(alphaP)	GP		inhibits					eIF2B	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_12841_s_158	9582312	( a) eIF2B reportedly does not catalyze GDP exchange on eIF2(alphaP) ( 15); ( b) eIF2(alphaP) displaces unphosphorylated eIF2 bound to eIF2B but unphosphorylated eIF2 does not ( 16); and ( c) eIF2(alphaP) inhibits the activity of eIF2B in the presence of low concentrations of substrate ( i.e. <10-fold molar excess of eIF2.GDP to eIF2(alphaP)) but at higher substrate concentrations the inhibition caused by eIF2(alphaP) is negligible ( 15), suggesting that eIF2(alphaP) is acting as a competitive inhibitor of eIF2B.	bind
1514	3	415	6	NULL	NULL	0	NULL	eIF2(alphaP)	GP		inhibit		competitively			eIF2B	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_12841_s_158	9582312	( a) eIF2B reportedly does not catalyze GDP exchange on eIF2(alphaP) ( 15); ( b) eIF2(alphaP) displaces unphosphorylated eIF2 bound to eIF2B but unphosphorylated eIF2 does not ( 16); and ( c) eIF2(alphaP) inhibits the activity of eIF2B in the presence of low concentrations of substrate ( i.e. <10-fold molar excess of eIF2.GDP to eIF2(alphaP)) but at higher substrate concentrations the inhibition caused by eIF2(alphaP) is negligible ( 15), suggesting that eIF2(alphaP) is acting as a competitive inhibitor of eIF2B.	bind
1516	4	415	6	NULL	NULL	0	NULL	eIF2B	GP		does not catalyze					GDP	Chemical	exchange of			NULL	on eIF2(alphaP)	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_12841_s_158	9582312	( a) eIF2B reportedly does not catalyze GDP exchange on eIF2(alphaP) ( 15); ( b) eIF2(alphaP) displaces unphosphorylated eIF2 bound to eIF2B but unphosphorylated eIF2 does not ( 16); and ( c) eIF2(alphaP) inhibits the activity of eIF2B in the presence of low concentrations of substrate ( i.e. <10-fold molar excess of eIF2.GDP to eIF2(alphaP)) but at higher substrate concentrations the inhibition caused by eIF2(alphaP) is negligible ( 15), suggesting that eIF2(alphaP) is acting as a competitive inhibitor of eIF2B.	bind
1517	5	415	6	NULL	NULL	0	NULL	Statement 2	Process		occurs in presence of					substrate	GP	low concentration			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_12841_s_158	9582312	( a) eIF2B reportedly does not catalyze GDP exchange on eIF2(alphaP) ( 15); ( b) eIF2(alphaP) displaces unphosphorylated eIF2 bound to eIF2B but unphosphorylated eIF2 does not ( 16); and ( c) eIF2(alphaP) inhibits the activity of eIF2B in the presence of low concentrations of substrate ( i.e. <10-fold molar excess of eIF2.GDP to eIF2(alphaP)) but at higher substrate concentrations the inhibition caused by eIF2(alphaP) is negligible ( 15), suggesting that eIF2(alphaP) is acting as a competitive inhibitor of eIF2B.	bind
1869	6	415	6	NULL	NULL	0	NULL	eIF2(alphaP)	GP		displaces					Statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_12841_s_158	9582312	( a) eIF2B reportedly does not catalyze GDP exchange on eIF2(alphaP) ( 15); ( b) eIF2(alphaP) displaces unphosphorylated eIF2 bound to eIF2B but unphosphorylated eIF2 does not ( 16); and ( c) eIF2(alphaP) inhibits the activity of eIF2B in the presence of low concentrations of substrate ( i.e. <10-fold molar excess of eIF2.GDP to eIF2(alphaP)) but at higher substrate concentrations the inhibition caused by eIF2(alphaP) is negligible ( 15), suggesting that eIF2(alphaP) is acting as a competitive inhibitor of eIF2B.	bind
1870	7	415	6	NULL	NULL	0	NULL	eIF2	GP	unphosphorylated	does not displace					Statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_12841_s_158	9582312	( a) eIF2B reportedly does not catalyze GDP exchange on eIF2(alphaP) ( 15); ( b) eIF2(alphaP) displaces unphosphorylated eIF2 bound to eIF2B but unphosphorylated eIF2 does not ( 16); and ( c) eIF2(alphaP) inhibits the activity of eIF2B in the presence of low concentrations of substrate ( i.e. <10-fold molar excess of eIF2.GDP to eIF2(alphaP)) but at higher substrate concentrations the inhibition caused by eIF2(alphaP) is negligible ( 15), suggesting that eIF2(alphaP) is acting as a competitive inhibitor of eIF2B.	bind
57935	1	416	5	NULL	NULL	0	NULL	eIF3	GP		bind					48S preinitiation complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_6_1381_s_257	14988734	( A) eIF4B, in concert with eIF4F (4E/4G/4A) or eIFiso4F, interacts with eIF3 bound to  the 48S preinitiation complex.	bind
57936	2	416	5	NULL	NULL	0	NULL	eIF4B	GP		interacts with					statement 1	GP				NULL		0	NULL	NULL	NULL	gw70_embo_23_6_1381_s_257	14988734	( A) eIF4B, in concert with eIF4F (4E/4G/4A) or eIFiso4F, interacts with eIF3 bound to  the 48S preinitiation complex.	bind
57937	3	416	5	NULL	NULL	0	NULL	eIF4F (4E/4G/4A)	GP		interacts with					statement 1	GP				NULL		0	NULL	NULL	NULL	gw70_embo_23_6_1381_s_257	14988734	( A) eIF4B, in concert with eIF4F (4E/4G/4A) or eIFiso4F, interacts with eIF3 bound to  the 48S preinitiation complex.	bind
57938	4	416	5	NULL	NULL	0	NULL	eIFiso4F	GP		interacts with					statement 1	GP				NULL		0	NULL	NULL	NULL	gw70_embo_23_6_1381_s_257	14988734	( A) eIF4B, in concert with eIF4F (4E/4G/4A) or eIFiso4F, interacts with eIF3 bound to  the 48S preinitiation complex.	bind
57939	5	416	5	NULL	NULL	0	NULL	statement 2	Process		in concert with					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_embo_23_6_1381_s_257	14988734	( A) eIF4B, in concert with eIF4F (4E/4G/4A) or eIFiso4F, interacts with eIF3 bound to  the 48S preinitiation complex.	bind
57940	6	416	5	NULL	NULL	0	NULL	statement 2	Process		in concert with					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_embo_23_6_1381_s_257	14988734	( A) eIF4B, in concert with eIF4F (4E/4G/4A) or eIFiso4F, interacts with eIF3 bound to  the 48S preinitiation complex.	bind
1518	1	416	6	NULL	NULL	0	NULL	eIF3	GP		bind					48S preinitiation complex	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_6_1381_s_257	14988734	( A) eIF4B, in concert with eIF4F (4E/4G/4A) or eIFiso4F, interacts with eIF3 bound to  the 48S preinitiation complex.	bind
1519	2	416	6	NULL	NULL	0	NULL	eIF4B	GP		interacts with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_6_1381_s_257	14988734	( A) eIF4B, in concert with eIF4F (4E/4G/4A) or eIFiso4F, interacts with eIF3 bound to  the 48S preinitiation complex.	bind
1520	3	416	6	NULL	NULL	0	NULL	eIF4F (4E/4G/4A)	GP		interacts with					Statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_6_1381_s_257	14988734	( A) eIF4B, in concert with eIF4F (4E/4G/4A) or eIFiso4F, interacts with eIF3 bound to  the 48S preinitiation complex.	bind
51778	4	416	6	NULL	NULL	0	NULL	eIFiso4F	GP		interacts with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_6_1381_s_257	14988734	( A) eIF4B, in concert with eIF4F (4E/4G/4A) or eIFiso4F, interacts with eIF3 bound to  the 48S preinitiation complex.	bind
51779	5	416	6	NULL	NULL	0	NULL	statement 2	Process		 in concert with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_6_1381_s_257	14988734	( A) eIF4B, in concert with eIF4F (4E/4G/4A) or eIFiso4F, interacts with eIF3 bound to  the 48S preinitiation complex.	bind
51780	6	416	6	NULL	NULL	0	NULL	statement 2	Process		in concert with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_6_1381_s_257	14988734	( A) eIF4B, in concert with eIF4F (4E/4G/4A) or eIFiso4F, interacts with eIF3 bound to  the 48S preinitiation complex.	bind
57941	1	421	5	NULL	NULL	0	NULL	DLX1	GP	recombinant	bind					Dlx5/ Dlx6 	GP			intergenic enhancer	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_32_3_884_s_172	14769946	( a) Electrophoretic mobility shift assays (EMSA) demonstrate recombinant DLX1 and DLX2  bind to the  Dlx5/ Dlx6 intergenic enhancer  in vitro.	bind
57942	2	421	5	NULL	NULL	0	NULL	DLX2	GP	recombinant	bind					Dlx5/ Dlx6	GP			intergenic enhancer	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_32_3_884_s_172	14769946	( a) Electrophoretic mobility shift assays (EMSA) demonstrate recombinant DLX1 and DLX2  bind to the  Dlx5/ Dlx6 intergenic enhancer  in vitro.	bind
1239	1	421	6	NULL	NULL	0	NULL	Dlx1	GP		bind					Dlx5/ Dlx6 	GP			intergenic enhancer	NULL	In vitro	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_32_3_884_s_172	14769946	( a) Electrophoretic mobility shift assays (EMSA) demonstrate recombinant DLX1 and DLX2  bind to the  Dlx5/ Dlx6 intergenic enhancer  in vitro.	bind
1240	2	421	6	NULL	NULL	0	NULL	DLX2	GP		bind					Dlx5/ Dlx6 	GP			intergenic enhancer	NULL	In vitro	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_32_3_884_s_172	14769946	( a) Electrophoretic mobility shift assays (EMSA) demonstrate recombinant DLX1 and DLX2  bind to the  Dlx5/ Dlx6 intergenic enhancer  in vitro.	bind
57943	1	423	5	NULL	NULL	0	NULL	Cdc20	GP		associates with					APC	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_24_3278_s_98	11751633	( A) Emi1 can bind Cdc20 and Cdh1 already associated with the APC.	bind
57944	2	423	5	NULL	NULL	0	NULL	Cdh1	GP		associates with					APC	GP				NULL		0	NULL	NULL	NULL	gw60_genesdev_15_24_3278_s_98	11751633	( A) Emi1 can bind Cdc20 and Cdh1 already associated with the APC.	bind
57945	3	423	5	NULL	NULL	0	NULL	Emi1	GP		bind					statement 1	GP				NULL		0	NULL	NULL	NULL	gw60_genesdev_15_24_3278_s_98	11751633	( A) Emi1 can bind Cdc20 and Cdh1 already associated with the APC.	bind
57946	4	423	5	NULL	NULL	0	NULL	Emi1	GP		bind					statement 1	GP				NULL		0	NULL	NULL	NULL	gw60_genesdev_15_24_3278_s_98	11751633	( A) Emi1 can bind Cdc20 and Cdh1 already associated with the APC.	bind
1282	1	423	6	NULL	NULL	0	NULL	Cdc20	GP		associates					APC	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_24_3278_s_98	11751633	( A) Emi1 can bind Cdc20 and Cdh1 already associated with the APC.	bind
1283	2	423	6	NULL	NULL	0	NULL	Cdh1	GP		associates					APC	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_24_3278_s_98	11751633	( A) Emi1 can bind Cdc20 and Cdh1 already associated with the APC.	bind
1285	4	423	6	NULL	NULL	0	NULL	Emi1	GP		bind					Statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_24_3278_s_98	11751633	( A) Emi1 can bind Cdc20 and Cdh1 already associated with the APC.	bind
1286	3	423	6	NULL	NULL	0	NULL	Emi1	GP		bind					Statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_24_3278_s_98	11751633	( A) Emi1 can bind Cdc20 and Cdh1 already associated with the APC.	bind
57947	1	425	5	NULL	NULL	0	NULL	p53	GP		bind					p53-responsive gene sequence	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_pnas_99_22_14548_s_109	12357032	( A) EMSA showing binding of p53 to a p53-responsive gene sequence.	bind
1289	1	425	6	NULL	NULL	0	NULL	p53	GP		bind					p53	GP			responsive gene sequence	NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_22_14548_s_109	12357032	( A) EMSA showing binding of p53 to a p53-responsive gene sequence.	bind
57948	1	426	5	NULL	NULL	0	NULL	RARalpha1deltaBC	GP	recombinant;;purified	does not bind					DR5	GP			RARE	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_4901_s_190	11812818	( A) EMSA using purified recombinant proteins (RARalpha1, RXRalpha and RARalpha1deltaBC) shows that RARalpha1deltaBC does not bind the RARE DR5 (lane 2), unlike RARalpha1 and RXRalpha (lanes 3 and 4, respectively).	bind
57949	2	426	5	NULL	NULL	0	NULL	RARalpha1	GP	recombinant;;purified	bind					DR5	GP			RARE	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_4901_s_190	11812818	( A) EMSA using purified recombinant proteins (RARalpha1, RXRalpha and RARalpha1deltaBC) shows that RARalpha1deltaBC does not bind the RARE DR5 (lane 2), unlike RARalpha1 and RXRalpha (lanes 3 and 4, respectively).	bind
57950	3	426	5	NULL	NULL	0	NULL	RXRalpha	GP	recombinant;;purified	bind					DR5	GP			RARE	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_4901_s_190	11812818	( A) EMSA using purified recombinant proteins (RARalpha1, RXRalpha and RARalpha1deltaBC) shows that RARalpha1deltaBC does not bind the RARE DR5 (lane 2), unlike RARalpha1 and RXRalpha (lanes 3 and 4, respectively).	bind
1291	1	426	6	NULL	NULL	0	NULL	RARalpha1deltaBC	GP	purified;;recombinant	does not bind					DR5	GP			RARE 	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_4901_s_190	11812818	( A) EMSA using purified recombinant proteins (RARalpha1, RXRalpha and RARalpha1deltaBC) shows that RARalpha1deltaBC does not bind the RARE DR5 (lane 2), unlike RARalpha1 and RXRalpha (lanes 3 and 4, respectively).	bind
1293	2	426	6	NULL	NULL	0	NULL	RXRalpha	GP		bind					DR5	GP			RARE 	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_4901_s_190	11812818	( A) EMSA using purified recombinant proteins (RARalpha1, RXRalpha and RARalpha1deltaBC) shows that RARalpha1deltaBC does not bind the RARE DR5 (lane 2), unlike RARalpha1 and RXRalpha (lanes 3 and 4, respectively).	bind
1294	3	426	6	NULL	NULL	0	NULL	RARalpha1	GP		bind					DR5	GP			RARE 	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_4901_s_190	11812818	( A) EMSA using purified recombinant proteins (RARalpha1, RXRalpha and RARalpha1deltaBC) shows that RARalpha1deltaBC does not bind the RARE DR5 (lane 2), unlike RARalpha1 and RXRalpha (lanes 3 and 4, respectively).	bind
57951	1	427	5	NULL	NULL	0	NULL	Apaf-1	GP	endogenous	bind					Apaf-1	GP		1-570		NULL		0	NULL	NULL	NULL	gw60_embo_18_13_3586_s_114	10393175	( A) Endogenous Apaf-1 binds Apaf-1(1-570) in the presence of cytochrome  c and dATP.	bind
57952	2	427	5	NULL	NULL	0	NULL	statement 1	Process		in the presence of					cytochrome c	GP				NULL		0	NULL	NULL	NULL	gw60_embo_18_13_3586_s_114	10393175	( A) Endogenous Apaf-1 binds Apaf-1(1-570) in the presence of cytochrome  c and dATP.	bind
57953	3	427	5	NULL	NULL	0	NULL	statement 1	GP	endogenous	in the presence of					dATP	Chemical				NULL		0	NULL	NULL	NULL	gw60_embo_18_13_3586_s_114	10393175	( A) Endogenous Apaf-1 binds Apaf-1(1-570) in the presence of cytochrome  c and dATP.	bind
1295	1	427	6	NULL	NULL	0	NULL	Apaf-1	GP	endogenous	bind					Apaf-1	GP		1-570		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_13_3586_s_114	10393175	( A) Endogenous Apaf-1 binds Apaf-1(1-570) in the presence of cytochrome  c and dATP.	bind
1296	2	427	6	NULL	NULL	0	NULL	Statement 1	Process		occurs in presence of					cytochrome c	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_13_3586_s_114	10393175	( A) Endogenous Apaf-1 binds Apaf-1(1-570) in the presence of cytochrome  c and dATP.	bind
1297	3	427	6	NULL	NULL	0	NULL	Statement 1	Process		occurs in presence of					dATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_13_3586_s_114	10393175	( A) Endogenous Apaf-1 binds Apaf-1(1-570) in the presence of cytochrome  c and dATP.	bind
57954	1	428	5	NULL	NULL	0	NULL	CREB	GP		bind					CART	GP			promoter	NULL		0	NULL	NULL	NULL	gw70_pnas_103_39_14489_s_93	16971488	( A) Estradiol increases CREB binding to CART promoter DNA.	bind
57955	2	428	5	NULL	NULL	0	NULL	Estradiol	GP		increases					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_103_39_14489_s_93	16971488	( A) Estradiol increases CREB binding to CART promoter DNA.	bind
1299	1	428	6	NULL	NULL	0	NULL	CREB	GP		bind					CART	GP			promoter DNA	NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_39_14489_s_93	16971488	( A) Estradiol increases CREB binding to CART promoter DNA.	bind
1300	2	428	6	NULL	NULL	0	NULL	Estradiol	Chemical		increases					Statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_39_14489_s_93	16971488	( A) Estradiol increases CREB binding to CART promoter DNA.	bind
57956	1	429	5	NULL	NULL	0	NULL	CITED1	GP		bind					ERalpha	GP				NULL		0	NULL	NULL	NULL	gw60_genesdev_15_19_2598_s_144	11581164	( A) Estrogen-dependent binding of CITED1 to ERalpha.	bind
57957	2	429	5	NULL	NULL	0	NULL	statement 1	Process		is dependent on					Estrogen	GP				NULL		0	NULL	NULL	NULL	gw60_genesdev_15_19_2598_s_144	11581164	( A) Estrogen-dependent binding of CITED1 to ERalpha.	bind
1302	1	429	6	NULL	NULL	0	NULL	CITED1	GP		bind					ERalpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_19_2598_s_144	11581164	( A) Estrogen-dependent binding of CITED1 to ERalpha.	bind
1303	2	429	6	NULL	NULL	0	NULL	Statement 1	Process		dependent on					Estrogen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_19_2598_s_144	11581164	( A) Estrogen-dependent binding of CITED1 to ERalpha.	bind
57958	1	430	5	NULL	NULL	0	NULL	Sema4D	GP		bind					plexin-B1	GP				NULL	COS-7 cells	0	NULL	NULL	NULL	gw60_genesdev_16_7_836_s_67	11937491	( A) Expression of RacL61 enhances the binding of Sema4D to plexin-B1 in COS-7 cells.	bind
57959	2	430	5	NULL	NULL	0	NULL	RacL61	GP	expression of	enhances					statement 1	Process				NULL	COS-7 cells	NULL	NULL	NULL	NULL	gw60_genesdev_16_7_836_s_67	11937491	( A) Expression of RacL61 enhances the binding of Sema4D to plexin-B1 in COS-7 cells.	bind
1306	1	430	6	NULL	NULL	0	NULL	Sema4D	GP		bind					plexin-B1	GP				NULL	Cos-7 cells	NULL	NULL	NULL	NULL	gw60_genesdev_16_7_836_s_67	11937491	( A) Expression of RacL61 enhances the binding of Sema4D to plexin-B1 in COS-7 cells.	bind
1308	2	430	6	NULL	NULL	0	NULL	RacL61	GP	expression of	enhances					Statement 1	Process				NULL	COS-7 cells	NULL	NULL	NULL	NULL	gw60_genesdev_16_7_836_s_67	11937491	( A) Expression of RacL61 enhances the binding of Sema4D to plexin-B1 in COS-7 cells.	bind
57960	1	434	5	NULL	NULL	0	NULL	scFv	GP		bind					BMS	Cell				NULL	human plasma	NULL	NULL	NULL	NULL	gw70_pnas_101_49_17210_s_166	15563590	( A) Flow cytometric analysis of scFv binding to BMS breast cancer cells in human plasma  anticoagulated with 50 nM PPACK.	bind
57961	2	434	5	NULL	NULL	0	NULL	BMS	Cell		is a type of					breast cancer cells	Cell				NULL		0	NULL	NULL	NULL	gw70_pnas_101_49_17210_s_166	15563590	( A) Flow cytometric analysis of scFv binding to BMS breast cancer cells in human plasma  anticoagulated with 50 nM PPACK.	bind
1310	1	434	6	NULL	NULL	0	NULL	scFv	GP		bind					BMS breast cancer cells	Cell				NULL	human plasma	NULL	NULL	NULL	NULL	gw70_pnas_101_49_17210_s_166	15563590	( A) Flow cytometric analysis of scFv binding to BMS breast cancer cells in human plasma  anticoagulated with 50 nM PPACK.	bind
57962	1	435	5	NULL	NULL	0	NULL	mAb 38C2	GP		bind					M21 cells	Cell				NULL		0	NULL	NULL	NULL	gw70_pnas_100_9_5396_s_92	12702756	( A) Flow cytometry histogram showing the binding of mAb 38C2 to human melanoma M21 cells  in the presence of a twice equimolar concentration of SCS-873 (red).	bind
57963	2	435	5	NULL	NULL	0	NULL	M21 cells	Cell		is a type of					human melanoma cells	Cell				NULL		0	NULL	NULL	NULL	gw70_pnas_100_9_5396_s_92	12702756	( A) Flow cytometry histogram showing the binding of mAb 38C2 to human melanoma M21 cells  in the presence of a twice equimolar concentration of SCS-873 (red).	bind
57964	3	435	5	NULL	NULL	0	NULL	statement 1	Process		in the presence of					SCS-873	Chemical				NULL		0	NULL	NULL	NULL	gw70_pnas_100_9_5396_s_92	12702756	( A) Flow cytometry histogram showing the binding of mAb 38C2 to human melanoma M21 cells  in the presence of a twice equimolar concentration of SCS-873 (red).	bind
1327	1	435	6	NULL	NULL	0	NULL	mAb 38C2	AminoAcid		bind					melanoma M21 cells	Cell	human			NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_9_5396_s_92	12702756	( A) Flow cytometry histogram showing the binding of mAb 38C2 to human melanoma M21 cells  in the presence of a twice equimolar concentration of SCS-873 (red).	bind
1328	2	435	6	NULL	NULL	0	NULL	Statement 1	Process		occurs in presence of					SCS-873	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_9_5396_s_92	12702756	( A) Flow cytometry histogram showing the binding of mAb 38C2 to human melanoma M21 cells  in the presence of a twice equimolar concentration of SCS-873 (red).	bind
57965	1	438	5	NULL	NULL	0	NULL	FMRP	GP		bind					MBP	GP			3''-UTR	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_11_2276_s_200	11376146	( A) FMRP binds to the MBP 3''-UTR.	bind
1329	1	438	6	NULL	NULL	0	NULL	FMRP	GP		bind					MBP	GP			3''-UTR	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_11_2276_s_200	11376146	( A) FMRP binds to the MBP 3''-UTR.	bind
57966	1	442	5	NULL	NULL	0	NULL	c-Myc	GP	full-length;;35S-labeled	bind					GST-cdr2					NULL	in vitro	0	NULL	NULL	NULL	gw60_genesdev_13_16_2087_s_47	10465786	( A) Full-length 35S-labeled c-Myc binds to GST-cdr2 in vitro.	bind
1330	1	442	6	NULL	NULL	0	NULL	c-Myc	GP	Full-length;;35S-labeled	bind					GST-cdr2	GP				NULL	In vitro	NULL	NULL	NULL	NULL	gw60_genesdev_13_16_2087_s_47	10465786	( A) Full-length 35S-labeled c-Myc binds to GST-cdr2 in vitro.	bind
57967	1	444	5	NULL	NULL	0	NULL	FWD1	GP		bind					Skp1	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_96_7_3859_s_73	10097128	( A) FWD1 binds to Skp1.	bind
1331	1	444	6	NULL	NULL	0	NULL	FWD1	GP		bind					Skp1	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_7_3859_s_73	10097128	( A) FWD1 binds to Skp1.	bind
57968	1	445	5	NULL	NULL	0	NULL	GA	GP		bind					TfR	GP				NULL	in vitro	0	NULL	NULL	NULL	gw70_pnas_102_34_12095_s_126	16103367	( A) GA binds TfR  in vitro.	bind
1332	1	445	6	NULL	NULL	0	NULL	GA	GP		bind					TfR	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_102_34_12095_s_126	16103367	( A) GA binds TfR  in vitro.	bind
57969	1	446	5	NULL	NULL	0	NULL	GA	GP		induce					Cbl	GP	phosphorylation of	tyrosine		NULL		0	NULL	NULL	NULL	gw70_pnas_103_30_11318_s_90	16844778	( A) GA induces Cbl tyrosine phosphorylation and PI3-kinase p85 binding to Cbl in an  Src-dependent manner.	bind
57970	2	446	5	NULL	NULL	0	NULL	PI3-kinase	GP		bind			p85		Cbl	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_103_30_11318_s_90	16844778	( A) GA induces Cbl tyrosine phosphorylation and PI3-kinase p85 binding to Cbl in an  Src-dependent manner.	bind
57971	3	446	5	NULL	NULL	0	NULL	GA	GP		induce					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_103_30_11318_s_90	16844778	( A) GA induces Cbl tyrosine phosphorylation and PI3-kinase p85 binding to Cbl in an  Src-dependent manner.	bind
57972	4	446	5	NULL	NULL	0	NULL	statement 1	Process		is dependent on					Src	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_103_30_11318_s_90	16844778	( A) GA induces Cbl tyrosine phosphorylation and PI3-kinase p85 binding to Cbl in an  Src-dependent manner.	bind
57973	5	446	5	NULL	NULL	0	NULL	statement 3	Process		is dependent on					Src	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_103_30_11318_s_90	16844778	( A) GA induces Cbl tyrosine phosphorylation and PI3-kinase p85 binding to Cbl in an  Src-dependent manner.	bind
1336	1	446	6	NULL	NULL	0	NULL	PI3-kinase p85	GP		bind					Cbl	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_30_11318_s_90	16844778	( A) GA induces Cbl tyrosine phosphorylation and PI3-kinase p85 binding to Cbl in an  Src-dependent manner.	bind
1337	2	446	6	NULL	NULL	0	NULL	GA	Chemical		induce					Cbl	GP	phosphorylation of	tyrosine		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_30_11318_s_90	16844778	( A) GA induces Cbl tyrosine phosphorylation and PI3-kinase p85 binding to Cbl in an  Src-dependent manner.	bind
1338	3	446	6	NULL	NULL	0	NULL	GA	Chemical		induce					Statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_30_11318_s_90	16844778	( A) GA induces Cbl tyrosine phosphorylation and PI3-kinase p85 binding to Cbl in an  Src-dependent manner.	bind
1339	4	446	6	NULL	NULL	0	NULL	Statement 1	Process		depend on					Src	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_30_11318_s_90	16844778	( A) GA induces Cbl tyrosine phosphorylation and PI3-kinase p85 binding to Cbl in an  Src-dependent manner.	bind
57974	1	448	5	NULL	NULL	0	NULL	GAPDH	GP		bind					Htt	GP				NULL	in vitro	0	NULL	NULL	NULL	gw70_pnas_103_9_3405_s_29	16492755	( A) GAPDH binds to Htt  in vitro.	bind
1340	1	448	6	NULL	NULL	0	NULL	GAPDH	GP		bind					Htt	GP				NULL	In vitro	NULL	NULL	NULL	NULL	gw70_pnas_103_9_3405_s_29	16492755	( A) GAPDH binds to Htt  in vitro.	bind
57978	1	449	5	NULL	NULL	0	NULL	nuclear extracts	CellComponent	zebrafish;;eye	bind					AP-1 oligonucleotides	GP	consensus			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_29_10194_s_51	16000406	( A) Gel mobility-shift assay of zebrafish eye nuclear extracts binding to consensus  AP-1 or CRE oligonucleotides.	bind
57979	2	449	5	NULL	NULL	0	NULL	nuclear extracts	CellComponent	zebrafish;;eye	bind					CRE oligonucleotides	GP	consensus			NULL		0	NULL	NULL	NULL	gw70_pnas_102_29_10194_s_51	16000406	( A) Gel mobility-shift assay of zebrafish eye nuclear extracts binding to consensus  AP-1 or CRE oligonucleotides.	bind
1341	1	449	6	NULL	NULL	0	NULL	eye nuclear extracts	OrganismPart	zebrafish	bind					consensus AP-1 oligonucleotides	NucleicAcid			site	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_29_10194_s_51	16000406	( A) Gel mobility-shift assay of zebrafish eye nuclear extracts binding to consensus  AP-1 or CRE oligonucleotides.	bind
1343	2	449	6	NULL	NULL	0	NULL	eye nuclear extracts	OrganismPart	zebrafish	bind					CRE oligonucleotides	NucleicAcid			site	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_29_10194_s_51	16000406	( A) Gel mobility-shift assay of zebrafish eye nuclear extracts binding to consensus  AP-1 or CRE oligonucleotides.	bind
57980	1	451	5	NULL	NULL	0	NULL	C/EBP	GP		bind					C/EBP-binding site	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_24_3_475_s_178	12663507	( A) Gel shift analysis of C/EBP binding to the C/EBP-binding site.	bind
1345	1	451	6	NULL	NULL	0	NULL	C/EBP	GP		bind						NucleicAcid			C/EBP-binding site	NULL		NULL	NULL	NULL	NULL	gw60_carcinogenesis_24_3_475_s_178	12663507	( A) Gel shift analysis of C/EBP binding to the C/EBP-binding site.	bind
57981	1	455	5	NULL	NULL	0	NULL	ChREBP	GP		bind					LPK	GP			ChRE	NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_44_15597_s_128	15496471	( A) Gel-shift analysis of ChREBP bound to ChREs of LPK, ACC1, and FAS.	bind
57982	2	455	5	NULL	NULL	0	NULL	ChREBP	GP		bind					ACC1	GP			ChRE	NULL		0	NULL	NULL	NULL	gw70_pnas_101_44_15597_s_128	15496471	( A) Gel-shift analysis of ChREBP bound to ChREs of LPK, ACC1, and FAS.	bind
57983	3	455	5	NULL	NULL	0	NULL	ChREBP	GP		bind					FAS	GP			ChRE	NULL		0	NULL	NULL	NULL	gw70_pnas_101_44_15597_s_128	15496471	( A) Gel-shift analysis of ChREBP bound to ChREs of LPK, ACC1, and FAS.	bind
1346	1	455	6	NULL	NULL	0	NULL	ChREBP	GP		bind					LPK	GP			ChRE	NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_44_15597_s_128	15496471	( A) Gel-shift analysis of ChREBP bound to ChREs of LPK, ACC1, and FAS.	bind
1347	2	455	6	NULL	NULL	0	NULL	ChREBP	GP		bind					ACC1	GP			ChRE	NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_44_15597_s_128	15496471	( A) Gel-shift analysis of ChREBP bound to ChREs of LPK, ACC1, and FAS.	bind
1348	3	455	6	NULL	NULL	0	NULL	ChREBP	GP		bind					FAS	GP			ChRE	NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_44_15597_s_128	15496471	( A) Gel-shift analysis of ChREBP bound to ChREs of LPK, ACC1, and FAS.	bind
57984	1	458	5	NULL	NULL	0	NULL	Gic2p	GP		bind					Cdc42p-GTP	GP				NULL		0	NULL	NULL	NULL	gw60_genesdev_11_22_2972_s_66	9367980	( A) Gic2p binds to Cdc42p-GTP.	bind
1349	1	458	6	NULL	NULL	0	NULL	Gic2p	GP		bind					Cdc42p-GTP	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_22_2972_s_66	9367980	( A) Gic2p binds to Cdc42p-GTP.	bind
57985	1	459	5	NULL	NULL	0	NULL	Gp33	GP		bind					RNAP	GP		core subunits		NULL		0	NULL	NULL	NULL	gw70_pnas_101_50_17365_s_83	15574501	( A) Gp33 binding to individual RNAP core subunits.	bind
1351	1	459	6	NULL	NULL	0	NULL	Gp33	GP		bind					 RNAP 	GP		individual core subunits		NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_50_17365_s_83	15574501	( A) Gp33 binding to individual RNAP core subunits.	bind
57986	1	460	5	NULL	NULL	0	NULL	GTP	Chemical		bind					heterotrimeric G proteins	GP	a subunit of			NULL		0	NULL	NULL	NULL	gw60_science_294_5548_1845_s_25	11729293	( A) GPCRs promote binding of GTP to the a subunit of heterotrimeric G proteins.	bind
57987	2	460	5	NULL	NULL	0	NULL	GPCRs	GP		promotes					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_science_294_5548_1845_s_25	11729293	( A) GPCRs promote binding of GTP to the a subunit of heterotrimeric G proteins.	bind
1354	1	460	6	NULL	NULL	0	NULL	GTP	Chemical		bind					heterotrimeric G proteins	GP		subunit		NULL		NULL	NULL	NULL	NULL	gw60_science_294_5548_1845_s_25	11729293	( A) GPCRs promote binding of GTP to the a subunit of heterotrimeric G proteins.	bind
1355	2	460	6	NULL	NULL	0	NULL	GPCRs	GP		promote					Statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_294_5548_1845_s_25	11729293	( A) GPCRs promote binding of GTP to the a subunit of heterotrimeric G proteins.	bind
57988	1	463	5	NULL	NULL	0	NULL	GST-Ebp1	GP		bind					HDAC	GP	activity of			NULL	Hela cells	0	NULL	NULL	NULL	gw60_nucleicacidsres_31_8_2168_s_201	12682367	( A) GST-Ebp1 binds HDAC activity from Hela cells.	bind
1356	1	463	6	NULL	NULL	0	NULL	GST-Ebp1	GP		bind					HDAC	GP				NULL	Hela cells	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_8_2168_s_201	12682367	( A) GST-Ebp1 binds HDAC activity from Hela cells.	bind
57989	1	465	5	NULL	NULL	0	NULL	stargazin	GP	point mutant	does not bind			T321F		PSD-95	GP	WT			NULL		0	NULL	NULL	NULL	gw60_pnas_99_21_13902_s_149	12359873	( A) GST-fusion proteins show that stargazin with a point mutation in its PDZ-binding region (T321F) does not bind WT PSD-95, but does bind PSD-95 bearing a compensatory point mutation (H225V) in its second PDZ domain.	bind
57990	2	465	5	NULL	NULL	0	NULL	stargazin	GP	point mutant	bind			T321F		PSD-95	GP	compensatory point mutant	H225V		NULL		0	NULL	NULL	NULL	gw60_pnas_99_21_13902_s_149	12359873	( A) GST-fusion proteins show that stargazin with a point mutation in its PDZ-binding region (T321F) does not bind WT PSD-95, but does bind PSD-95 bearing a compensatory point mutation (H225V) in its second PDZ domain.	bind
1357	1	465	6	NULL	NULL	0	NULL	stargazin	GP	mutant	does not bind			 PDZ-binding region (T321F)		PSD-95	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_21_13902_s_149	12359873	( A) GST-fusion proteins show that stargazin with a point mutation in its PDZ-binding region (T321F) does not bind WT PSD-95, but does bind PSD-95 bearing a compensatory point mutation (H225V) in its second PDZ domain.	bind
1359	2	465	6	NULL	NULL	0	NULL	stargazin	GP	mutant	bind			 PDZ-binding region (T321F)		PSD-95	GP	mutant	 PDZ domain (H225V)		NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_21_13902_s_149	12359873	( A) GST-fusion proteins show that stargazin with a point mutation in its PDZ-binding region (T321F) does not bind WT PSD-95, but does bind PSD-95 bearing a compensatory point mutation (H225V) in its second PDZ domain.	bind
57991	1	469	5	NULL	NULL	0	NULL	Hesx1	GP		bind					TLE family corepressors	GP				NULL		0	NULL	NULL	NULL	gw60_genesdev_15_23_3193_s_104	11731482	( A) Hesx1 binds TLE family corepressors.	bind
1362	1	469	6	NULL	NULL	0	NULL	Hesx1	GP		bind					TLE family corepressors	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_23_3193_s_104	11731482	( A) Hesx1 binds TLE family corepressors.	bind
57992	1	471	5	NULL	NULL	0	NULL	His6CED-9	GP		bind			(68-251; G169E)		GST-CED-4	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_97_22_11916_s_75	11027303	( A) His6CED-9(68-251; G169E) binds GST-CED-4 as well as His6CED-9(68-251).	bind
57993	2	471	5	NULL	NULL	0	NULL	His6CED-9	GP		bind			(68-251; G169E)		His6CED-9	GP		(68-251)		NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_22_11916_s_75	11027303	( A) His6CED-9(68-251; G169E) binds GST-CED-4 as well as His6CED-9(68-251).	bind
1521	1	471	6	NULL	NULL	0	NULL	His6CED-9	GP		bind			68-251; G169E		GST-CED-4	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_22_11916_s_75	11027303	( A) His6CED-9(68-251; G169E) binds GST-CED-4 as well as His6CED-9(68-251).	bind
1522	2	471	6	NULL	NULL	0	NULL	His6CED-9	GP		bind			(68-251; G169E)		His6CED-9	GP		(68-251)		NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_22_11916_s_75	11027303	( A) His6CED-9(68-251; G169E) binds GST-CED-4 as well as His6CED-9(68-251).	bind
57994	1	474	5	NULL	NULL	0	NULL	HTm4	GP		bind					KAP-CDK2	GP				NULL		0	NULL	NULL	NULL	gw60_jclininvest_109_1_51_s_186	11781350	( a) HTm4 binds to KAP-CDK2 under normal physiological conditions.	bind
1523	1	474	6	NULL	NULL	0	NULL	HTm4	GP		bind					KAP-CDK2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_109_1_51_s_186	11781350	( a) HTm4 binds to KAP-CDK2 under normal physiological conditions.	bind
57995	1	475	5	NULL	NULL	0	NULL	Cds1	GP		bind					GST:Wee170	GP				NULL		0	NULL	NULL	NULL	gw60_science_280_5365_909_s_110	9572736	( A) HU stimulates Cds1 binding to GST:Wee170.	bind
57996	2	475	5	NULL	NULL	0	NULL	HU	Chemical		stimulates					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_science_280_5365_909_s_110	9572736	( A) HU stimulates Cds1 binding to GST:Wee170.	bind
1524	1	475	6	NULL	NULL	0	NULL	Cds1	GP		bind					GST:Wee170	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_280_5365_909_s_110	9572736	( A) HU stimulates Cds1 binding to GST:Wee170.	bind
1525	2	475	6	NULL	NULL	0	NULL	HU	GP		stimulates					Statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_280_5365_909_s_110	9572736	( A) HU stimulates Cds1 binding to GST:Wee170.	bind
57997	1	477	5	NULL	NULL	0	NULL	PABP	GP	human	does not bind			RRM2		eIF4G	GP	yeast			NULL		0	NULL	NULL	NULL	gw60_embo_18_11_3153_s_284	10357826	( A) Human PABP RRM2 cannot bind to yeast eIF4G.	bind
1526	1	477	6	NULL	NULL	0	NULL	PABP	GP	human	does not bind			RRM2		eIF4G	GP	yeast			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_11_3153_s_284	10357826	( A) Human PABP RRM2 cannot bind to yeast eIF4G.	bind
57998	1	478	5	NULL	NULL	0	NULL	PAHX	GP	human	bind		specifically			FKBP52	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_pnas_96_5_2104_s_149	10051602	( A) Human PAHX specifically binds FKBP52  in vitro.	bind
1527	1	478	6	NULL	NULL	0	NULL	PAHX	GP	human	bind		specifically			FKBP52	GP				NULL	In vitro	NULL	NULL	NULL	NULL	gw60_pnas_96_5_2104_s_149	10051602	( A) Human PAHX specifically binds FKBP52  in vitro.	bind
57999	1	479	5	NULL	NULL	0	NULL	VHL	GP	human	bind					peptide substrates	GP	hydroxylated			NULL		0	NULL	NULL	NULL	gw60_science_294_5545_1337_s_80	11598268	( A) Human VHL binds to all hydroxylated peptide substrates.	bind
1528	1	479	6	NULL	NULL	0	NULL	VHL	GP	human	bind					peptide substrate	GP	hydroxylated			NULL		NULL	NULL	NULL	NULL	gw60_science_294_5545_1337_s_80	11598268	( A) Human VHL binds to all hydroxylated peptide substrates.	bind
58000	1	486	5	NULL	NULL	0	NULL				bind				IGR	Clr3-myc/high H3K14Ac	GP				NULL	clr3delta	NULL	NULL	NULL	NULL	gw70_embo_24_16_2906_s_181	16079916	( A) IGR binding of Clr3-myc/high H3K14Ac in  clr3delta; ( B) ORF binding of Clr3-myc high H3K14Ac in  clr3delta; ( C) IGR binding of Sir2-myc/H3K9Ac in  sir2delta; ( D) ORF binding of Sir2-myc/high H3K9Ac in  sir2delta.	bind
58001	2	486	5	NULL	NULL	0	NULL				bind				ORF	Clr3-myc high H3K14Ac	GP				NULL	clr3delta	NULL	NULL	NULL	NULL	gw70_embo_24_16_2906_s_181	16079916	( A) IGR binding of Clr3-myc/high H3K14Ac in  clr3delta; ( B) ORF binding of Clr3-myc high H3K14Ac in  clr3delta; ( C) IGR binding of Sir2-myc/H3K9Ac in  sir2delta; ( D) ORF binding of Sir2-myc/high H3K9Ac in  sir2delta.	bind
58002	3	486	5	NULL	NULL	0	NULL				bind				IGR	Sir2-myc/H3K9Ac	GP				NULL	sir2delta	0	NULL	NULL	NULL	gw70_embo_24_16_2906_s_181	16079916	( A) IGR binding of Clr3-myc/high H3K14Ac in  clr3delta; ( B) ORF binding of Clr3-myc high H3K14Ac in  clr3delta; ( C) IGR binding of Sir2-myc/H3K9Ac in  sir2delta; ( D) ORF binding of Sir2-myc/high H3K9Ac in  sir2delta.	bind
58003	4	486	5	NULL	NULL	0	NULL				bind				ORF	Sir2-myc/high H3K9Ac	GP				NULL	sir2delta	0	NULL	NULL	NULL	gw70_embo_24_16_2906_s_181	16079916	( A) IGR binding of Clr3-myc/high H3K14Ac in  clr3delta; ( B) ORF binding of Clr3-myc high H3K14Ac in  clr3delta; ( C) IGR binding of Sir2-myc/H3K9Ac in  sir2delta; ( D) ORF binding of Sir2-myc/high H3K9Ac in  sir2delta.	bind
1529	1	486	6	NULL	NULL	0	NULL		NucleicAcid		bind				IGR	Clr3-myc/high H3K14Ac	GP				NULL	clr3delta	NULL	NULL	NULL	NULL	gw70_embo_24_16_2906_s_181	16079916	( A) IGR binding of Clr3-myc/high H3K14Ac in  clr3delta; ( B) ORF binding of Clr3-myc high H3K14Ac in  clr3delta; ( C) IGR binding of Sir2-myc/H3K9Ac in  sir2delta; ( D) ORF binding of Sir2-myc/high H3K9Ac in  sir2delta.	bind
1530	2	486	6	NULL	NULL	0	NULL		NucleicAcid		bind				ORF	Clr3-myc high H3K14Ac	GP				NULL	clr3delta	NULL	NULL	NULL	NULL	gw70_embo_24_16_2906_s_181	16079916	( A) IGR binding of Clr3-myc/high H3K14Ac in  clr3delta; ( B) ORF binding of Clr3-myc high H3K14Ac in  clr3delta; ( C) IGR binding of Sir2-myc/H3K9Ac in  sir2delta; ( D) ORF binding of Sir2-myc/high H3K9Ac in  sir2delta.	bind
1531	3	486	6	NULL	NULL	0	NULL		NucleicAcid		bind				IGR	Sir2-myc/H3K9Ac	GP				NULL	sir2delta	NULL	NULL	NULL	NULL	gw70_embo_24_16_2906_s_181	16079916	( A) IGR binding of Clr3-myc/high H3K14Ac in  clr3delta; ( B) ORF binding of Clr3-myc high H3K14Ac in  clr3delta; ( C) IGR binding of Sir2-myc/H3K9Ac in  sir2delta; ( D) ORF binding of Sir2-myc/high H3K9Ac in  sir2delta.	bind
1532	4	486	6	NULL	NULL	0	NULL		NucleicAcid		bind				ORF	Sir2-myc/high H3K9Ac	GP				NULL	sir2delta	NULL	NULL	NULL	NULL	gw70_embo_24_16_2906_s_181	16079916	( A) IGR binding of Clr3-myc/high H3K14Ac in  clr3delta; ( B) ORF binding of Clr3-myc high H3K14Ac in  clr3delta; ( C) IGR binding of Sir2-myc/H3K9Ac in  sir2delta; ( D) ORF binding of Sir2-myc/high H3K9Ac in  sir2delta.	bind
58004	1	487	5	NULL	NULL	0	NULL	clathrin-adaptor	GP		bind					GST-CI-MPR	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_97_16_9047_s_97	10908666	( A) Immunoblot analysis of clathrin-adaptor binding to GST-CI-MPR constructs confirms the recognition of tyrosine and/or dileucine motifs by AP-1 and AP-2.	bind
58005	2	487	5	NULL	NULL	0	NULL	AP-1	GP		recognizes								tyrosine;;dileucine motifs		NULL		0	NULL	NULL	NULL	gw60_pnas_97_16_9047_s_97	10908666	( A) Immunoblot analysis of clathrin-adaptor binding to GST-CI-MPR constructs confirms the recognition of tyrosine and/or dileucine motifs by AP-1 and AP-2.	bind
58006	3	487	5	NULL	NULL	0	NULL	AP-2	GP		recognizes								tyrosine;;dileucine motifs		NULL		0	NULL	NULL	NULL	gw60_pnas_97_16_9047_s_97	10908666	( A) Immunoblot analysis of clathrin-adaptor binding to GST-CI-MPR constructs confirms the recognition of tyrosine and/or dileucine motifs by AP-1 and AP-2.	bind
58007	4	487	5	NULL	NULL	0	NULL	statement 1	Process		confirms					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_97_16_9047_s_97	10908666	( A) Immunoblot analysis of clathrin-adaptor binding to GST-CI-MPR constructs confirms the recognition of tyrosine and/or dileucine motifs by AP-1 and AP-2.	bind
58008	5	487	5	NULL	NULL	0	NULL	statement 1	Process		confirms					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_97_16_9047_s_97	10908666	( A) Immunoblot analysis of clathrin-adaptor binding to GST-CI-MPR constructs confirms the recognition of tyrosine and/or dileucine motifs by AP-1 and AP-2.	bind
1533	1	487	6	NULL	NULL	0	NULL	clathrin-adaptor 	GP		bind					GST-CI-MPR	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_16_9047_s_97	10908666	( A) Immunoblot analysis of clathrin-adaptor binding to GST-CI-MPR constructs confirms the recognition of tyrosine and/or dileucine motifs by AP-1 and AP-2.	bind
1534	2	487	6	NULL	NULL	0	NULL	AP1	GP		recognizes						AminoAcid		tyrosine and/or dileucine motifs		NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_16_9047_s_97	10908666	( A) Immunoblot analysis of clathrin-adaptor binding to GST-CI-MPR constructs confirms the recognition of tyrosine and/or dileucine motifs by AP-1 and AP-2.	bind
1535	3	487	6	NULL	NULL	0	NULL	AP2	GP		recognizes						AminoAcid		tyrosine and/or dileucine motifs		NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_16_9047_s_97	10908666	( A) Immunoblot analysis of clathrin-adaptor binding to GST-CI-MPR constructs confirms the recognition of tyrosine and/or dileucine motifs by AP-1 and AP-2.	bind
1536	4	487	6	NULL	NULL	0	NULL	Statement 1	Process		confirms					Statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_16_9047_s_97	10908666	( A) Immunoblot analysis of clathrin-adaptor binding to GST-CI-MPR constructs confirms the recognition of tyrosine and/or dileucine motifs by AP-1 and AP-2.	bind
1537	5	487	6	NULL	NULL	0	NULL	Statement 1	Process		confirms					Statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_16_9047_s_97	10908666	( A) Immunoblot analysis of clathrin-adaptor binding to GST-CI-MPR constructs confirms the recognition of tyrosine and/or dileucine motifs by AP-1 and AP-2.	bind
58009	1	491	5	NULL	NULL	0	NULL	gD	GP	soluble	bind					GST-PFD	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_102_26_9323_s_166	15972328	( A) Immunoblots of soluble forms of gD bound by GST-PFD fusion proteins.	bind
58010	2	491	5	NULL	NULL	0	NULL	GST-PFD	GP		is a type of					fusion protein	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_102_26_9323_s_166	15972328	( A) Immunoblots of soluble forms of gD bound by GST-PFD fusion proteins.	bind
1538	1	491	6	NULL	NULL	0	NULL	gD	GP	soluble	bind					GST-PFD	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_26_9323_s_166	15972328	( A) Immunoblots of soluble forms of gD bound by GST-PFD fusion proteins.	bind
51782	2	491	6	NULL	NULL	0	NULL	GST-PFD	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_26_9323_s_166	15972328	( A) Immunoblots of soluble forms of gD bound by GST-PFD fusion proteins.	bind
58011	1	492	5	NULL	NULL	0	NULL	calstabin2	GP		bind			D37V		RyR2	GP		S2808D		NULL		0	NULL	NULL	NULL	gw70_pnas_103_9_3456_s_73	16481613	( A) Immunoblots showing that calstabin2 - D37V bound to RyR2 - S2808D (which mimics  chronically PKA-phosphorylated RyR2), whereas WT calstabin2 and mutants F36Y and  F99Y did not.	bind
58012	2	492	5	NULL	NULL	0	NULL	calstabin2	GP	WT	does not bind					RyR2	GP		S2808D		NULL		0	NULL	NULL	NULL	gw70_pnas_103_9_3456_s_73	16481613	( A) Immunoblots showing that calstabin2 - D37V bound to RyR2 - S2808D (which mimics  chronically PKA-phosphorylated RyR2), whereas WT calstabin2 and mutants F36Y and  F99Y did not.	bind
58013	3	492	5	NULL	NULL	0	NULL	calstabin2	GP	mutant	does not bind			F36Y 		RyR2	GP		S2808D		NULL		0	NULL	NULL	NULL	gw70_pnas_103_9_3456_s_73	16481613	( A) Immunoblots showing that calstabin2 - D37V bound to RyR2 - S2808D (which mimics  chronically PKA-phosphorylated RyR2), whereas WT calstabin2 and mutants F36Y and  F99Y did not.	bind
58014	4	492	5	NULL	NULL	0	NULL	calstabin2	GP	mutant	does not bind			F99Y		RyR2	GP		S2808D		NULL		0	NULL	NULL	NULL	gw70_pnas_103_9_3456_s_73	16481613	( A) Immunoblots showing that calstabin2 - D37V bound to RyR2 - S2808D (which mimics  chronically PKA-phosphorylated RyR2), whereas WT calstabin2 and mutants F36Y and  F99Y did not.	bind
58015	5	492	5	NULL	NULL	0	NULL	PKA	GP		phosphorylates					RyR2	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_103_9_3456_s_73	16481613	( A) Immunoblots showing that calstabin2 - D37V bound to RyR2 - S2808D (which mimics  chronically PKA-phosphorylated RyR2), whereas WT calstabin2 and mutants F36Y and  F99Y did not.	bind
58016	6	492	5	NULL	NULL	0	NULL	RyR2	GP		mimics		chronically	S2808D		statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_103_9_3456_s_73	16481613	( A) Immunoblots showing that calstabin2 - D37V bound to RyR2 - S2808D (which mimics  chronically PKA-phosphorylated RyR2), whereas WT calstabin2 and mutants F36Y and  F99Y did not.	bind
1539	1	492	6	NULL	NULL	0	NULL	calstabin2	GP		bind			D37V		RyR2	GP		S2808D		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_9_3456_s_73	16481613	( A) Immunoblots showing that calstabin2 - D37V bound to RyR2 - S2808D (which mimics  chronically PKA-phosphorylated RyR2), whereas WT calstabin2 and mutants F36Y and  F99Y did not.	bind
1540	2	492	6	NULL	NULL	0	NULL	calstabin2	GP	wild type	does not bind					RyR2	GP		S2808D		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_9_3456_s_73	16481613	( A) Immunoblots showing that calstabin2 - D37V bound to RyR2 - S2808D (which mimics  chronically PKA-phosphorylated RyR2), whereas WT calstabin2 and mutants F36Y and  F99Y did not.	bind
1541	3	492	6	NULL	NULL	0	NULL	calstabin2	GP	mutant	does not bind			F36Y		RyR2	GP		S2808D		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_9_3456_s_73	16481613	( A) Immunoblots showing that calstabin2 - D37V bound to RyR2 - S2808D (which mimics  chronically PKA-phosphorylated RyR2), whereas WT calstabin2 and mutants F36Y and  F99Y did not.	bind
1542	4	492	6	NULL	NULL	0	NULL	calstabin2	GP	mutant	does not bind			F99Y		RyR2	GP		S2808D		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_9_3456_s_73	16481613	( A) Immunoblots showing that calstabin2 - D37V bound to RyR2 - S2808D (which mimics  chronically PKA-phosphorylated RyR2), whereas WT calstabin2 and mutants F36Y and  F99Y did not.	bind
1543	6	492	6	NULL	NULL	0	NULL	RyR2	GP		mimics 		chronically	S2808D		statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_9_3456_s_73	16481613	( A) Immunoblots showing that calstabin2 - D37V bound to RyR2 - S2808D (which mimics  chronically PKA-phosphorylated RyR2), whereas WT calstabin2 and mutants F36Y and  F99Y did not.	bind
51783	5	492	6	NULL	NULL	0	NULL	PKA	GP		phosphorylate					RyR2	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_9_3456_s_73	16481613	( A) Immunoblots showing that calstabin2 - D37V bound to RyR2 - S2808D (which mimics  chronically PKA-phosphorylated RyR2), whereas WT calstabin2 and mutants F36Y and  F99Y did not.	bind
58017	1	494	5	NULL	NULL	0	NULL	SecA	GP	cytoplasmic				C-domain		SecA	GP	cytoplasmic	N-domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_16_13724_s_342	11825907	( a) In cytoplasmic SecA, binding of the C-domain to the N-domain represses both ATP hydrolysis and preprotein binding.	bind
58018	2	494	5	NULL	NULL	0	NULL	statement 1	Process		repress					ATP hydrolysis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_16_13724_s_342	11825907	( a) In cytoplasmic SecA, binding of the C-domain to the N-domain represses both ATP hydrolysis and preprotein binding.	bind
58019	3	494	5	NULL	NULL	0	NULL	statement 1	Process		repress					preprotein binding	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_16_13724_s_342	11825907	( a) In cytoplasmic SecA, binding of the C-domain to the N-domain represses both ATP hydrolysis and preprotein binding.	bind
1544	1	494	6	NULL	NULL	0	NULL		AminoAcid		bind			C-domain			AminoAcid		N-domain		NULL	cytoplasmic SecA	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_16_13724_s_342	11825907	( a) In cytoplasmic SecA, binding of the C-domain to the N-domain represses both ATP hydrolysis and preprotein binding.	bind
1545	2	494	6	NULL	NULL	0	NULL	Statement 1	Process		repress					ATP	Chemical	hydrolysis of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_16_13724_s_342	11825907	( a) In cytoplasmic SecA, binding of the C-domain to the N-domain represses both ATP hydrolysis and preprotein binding.	bind
1546	3	494	6	NULL	NULL	0	NULL	Statement 1	Process		repress					preprotein	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_16_13724_s_342	11825907	( a) In cytoplasmic SecA, binding of the C-domain to the N-domain represses both ATP hydrolysis and preprotein binding.	bind
58020	1	496	5	NULL	NULL	0	NULL	adenosine nucleotide	NucleicAcid		bind					NifL	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_46_16316_s_182	15534211	( A) In the absence of 2-oxoglutarate, both the reduced and oxidized forms of NifL inhibit  the activity of NifA, provided that adenosine nucleotide is bound to NifL ( ,  ,  ).	bind
58021	2	496	5	NULL	NULL	0	NULL	NifL	GP	oxidized	inhibits					NifA	GP	activity of			NULL		0	NULL	NULL	NULL	gw70_pnas_101_46_16316_s_182	15534211	( A) In the absence of 2-oxoglutarate, both the reduced and oxidized forms of NifL inhibit  the activity of NifA, provided that adenosine nucleotide is bound to NifL ( ,  ,  ).	bind
58022	3	496	5	NULL	NULL	0	NULL	statement 2	Process		in the absence of					2-oxoglutarate	Chemical				NULL		0	NULL	NULL	NULL	gw70_pnas_101_46_16316_s_182	15534211	( A) In the absence of 2-oxoglutarate, both the reduced and oxidized forms of NifL inhibit  the activity of NifA, provided that adenosine nucleotide is bound to NifL ( ,  ,  ).	bind
58023	4	496	5	NULL	NULL	0	NULL	NifL	GP	reduced	inhibit					NifA	GP	activity of			NULL		0	NULL	NULL	NULL	gw70_pnas_101_46_16316_s_182	15534211	( A) In the absence of 2-oxoglutarate, both the reduced and oxidized forms of NifL inhibit  the activity of NifA, provided that adenosine nucleotide is bound to NifL ( ,  ,  ).	bind
58024	5	496	5	NULL	NULL	0	NULL	statement 4	Process		in the absence of					2-oxoglutarate	Chemical				NULL		0	NULL	NULL	NULL	gw70_pnas_101_46_16316_s_182	15534211	( A) In the absence of 2-oxoglutarate, both the reduced and oxidized forms of NifL inhibit  the activity of NifA, provided that adenosine nucleotide is bound to NifL ( ,  ,  ).	bind
58025	6	496	5	NULL	NULL	0	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_46_16316_s_182	15534211	( A) In the absence of 2-oxoglutarate, both the reduced and oxidized forms of NifL inhibit  the activity of NifA, provided that adenosine nucleotide is bound to NifL ( ,  ,  ).	bind
58026	7	496	5	NULL	NULL	0	NULL	statement 1	Process		leads to					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_101_46_16316_s_182	15534211	( A) In the absence of 2-oxoglutarate, both the reduced and oxidized forms of NifL inhibit  the activity of NifA, provided that adenosine nucleotide is bound to NifL ( ,  ,  ).	bind
1551	1	496	6	NULL	NULL	0	NULL	adenosine nucleotide	NucleicAcid		bind					NifL	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_46_16316_s_182	15534211	( A) In the absence of 2-oxoglutarate, both the reduced and oxidized forms of NifL inhibit  the activity of NifA, provided that adenosine nucleotide is bound to NifL ( ,  ,  ).	bind
1552	3	496	6	NULL	NULL	0	NULL	NifL	GP	reduced	inhibit 					NifA	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_46_16316_s_182	15534211	( A) In the absence of 2-oxoglutarate, both the reduced and oxidized forms of NifL inhibit  the activity of NifA, provided that adenosine nucleotide is bound to NifL ( ,  ,  ).	bind
1553	2	496	6	NULL	NULL	0	NULL	NifL	GP	oxidized	inhibit					NifA	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_46_16316_s_182	15534211	( A) In the absence of 2-oxoglutarate, both the reduced and oxidized forms of NifL inhibit  the activity of NifA, provided that adenosine nucleotide is bound to NifL ( ,  ,  ).	bind
1582	4	496	6	NULL	NULL	0	NULL	statement 2	Process		occurs in absence of					2-oxoglutarate	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_46_16316_s_182	15534211	( A) In the absence of 2-oxoglutarate, both the reduced and oxidized forms of NifL inhibit  the activity of NifA, provided that adenosine nucleotide is bound to NifL ( ,  ,  ).	bind
1589	5	496	6	NULL	NULL	0	NULL	Statement 3	Process		occurs in absence of					2-oxoglutarate	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_46_16316_s_182	15534211	( A) In the absence of 2-oxoglutarate, both the reduced and oxidized forms of NifL inhibit  the activity of NifA, provided that adenosine nucleotide is bound to NifL ( ,  ,  ).	bind
1593	6	496	6	NULL	NULL	0	NULL	statement 2	Process		dependent on					Statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_46_16316_s_182	15534211	( A) In the absence of 2-oxoglutarate, both the reduced and oxidized forms of NifL inhibit  the activity of NifA, provided that adenosine nucleotide is bound to NifL ( ,  ,  ).	bind
1594	7	496	6	NULL	NULL	0	NULL	Statement 3	Process		dependent on					Statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_46_16316_s_182	15534211	( A) In the absence of 2-oxoglutarate, both the reduced and oxidized forms of NifL inhibit  the activity of NifA, provided that adenosine nucleotide is bound to NifL ( ,  ,  ).	bind
58027	1	498	5	NULL	NULL	0	NULL	GST-BAK	GP		bind					BCL-XL	GP	IVT			NULL	in vitro	0	NULL	NULL	NULL	gw60_genesdev_14_16_2060_s_136	10950869	( A) In vitro binding between GST-BAK and IVT BCL-XL, p15 BID, and BIDalpha345/TM, but not p15 BID mIII.4 or BIDalpha345/TM mIII.4 (lanes  1-5).	bind
58028	2	498	5	NULL	NULL	0	NULL	GST-BAK	GP		bind					p15 BID	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_genesdev_14_16_2060_s_136	10950869	( A) In vitro binding between GST-BAK and IVT BCL-XL, p15 BID, and BIDalpha345/TM, but not p15 BID mIII.4 or BIDalpha345/TM mIII.4 (lanes  1-5).	bind
58029	3	498	5	NULL	NULL	0	NULL	GST-BAK	GP		bind					BIDalpha345/TM	GP				NULL	in vitro	0	NULL	NULL	NULL	gw60_genesdev_14_16_2060_s_136	10950869	( A) In vitro binding between GST-BAK and IVT BCL-XL, p15 BID, and BIDalpha345/TM, but not p15 BID mIII.4 or BIDalpha345/TM mIII.4 (lanes  1-5).	bind
58030	4	498	5	NULL	NULL	0	NULL	GST-BAK	GP		does not bind					p15 BID mIII.4	GP				NULL	in vitro	0	NULL	NULL	NULL	gw60_genesdev_14_16_2060_s_136	10950869	( A) In vitro binding between GST-BAK and IVT BCL-XL, p15 BID, and BIDalpha345/TM, but not p15 BID mIII.4 or BIDalpha345/TM mIII.4 (lanes  1-5).	bind
58031	5	498	5	NULL	NULL	0	NULL	GST-BAK	GP		does not bind					BIDalpha345/TM mIII.4	GP				NULL	in vitro	0	NULL	NULL	NULL	gw60_genesdev_14_16_2060_s_136	10950869	( A) In vitro binding between GST-BAK and IVT BCL-XL, p15 BID, and BIDalpha345/TM, but not p15 BID mIII.4 or BIDalpha345/TM mIII.4 (lanes  1-5).	bind
1895	1	498	6	NULL	NULL	0	NULL	GST-BAK	GP		bind					BCL-XL	GP	IVT			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_genesdev_14_16_2060_s_136	10950869	( A) In vitro binding between GST-BAK and IVT BCL-XL, p15 BID, and BIDalpha345/TM, but not p15 BID mIII.4 or BIDalpha345/TM mIII.4 (lanes  1-5).	bind
1896	2	498	6	NULL	NULL	0	NULL	GST-BAK	GP		bind					p15 BID	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_genesdev_14_16_2060_s_136	10950869	( A) In vitro binding between GST-BAK and IVT BCL-XL, p15 BID, and BIDalpha345/TM, but not p15 BID mIII.4 or BIDalpha345/TM mIII.4 (lanes  1-5).	bind
1897	3	498	6	NULL	NULL	0	NULL	GST-BAK	GP		bind					BIDalpha345/TM	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_genesdev_14_16_2060_s_136	10950869	( A) In vitro binding between GST-BAK and IVT BCL-XL, p15 BID, and BIDalpha345/TM, but not p15 BID mIII.4 or BIDalpha345/TM mIII.4 (lanes  1-5).	bind
1898	4	498	6	NULL	NULL	0	NULL	GST-BAK	GP		does not bind					p15 BID mIII.4	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_genesdev_14_16_2060_s_136	10950869	( A) In vitro binding between GST-BAK and IVT BCL-XL, p15 BID, and BIDalpha345/TM, but not p15 BID mIII.4 or BIDalpha345/TM mIII.4 (lanes  1-5).	bind
1899	5	498	6	NULL	NULL	0	NULL	GST-BAK	GP		does not bind					BIDalpha345/TM mIII.4	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_genesdev_14_16_2060_s_136	10950869	( A) In vitro binding between GST-BAK and IVT BCL-XL, p15 BID, and BIDalpha345/TM, but not p15 BID mIII.4 or BIDalpha345/TM mIII.4 (lanes  1-5).	bind
58032	1	499	5	NULL	NULL	0	NULL	Eps15	GP		bind					EH-binding proteins	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_genesdev_11_17_2239_s_102	9303539	( A) In vitro binding of Eps15 to Gst fusions of EH-binding proteins.	bind
58033	2	499	5	NULL	NULL	0	NULL	EH-binding proteins	GP		is a type of					GST fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_17_2239_s_102	9303539	( A) In vitro binding of Eps15 to Gst fusions of EH-binding proteins.	bind
1596	1	499	6	NULL	NULL	0	NULL	Eps15	GP		bind					EH-binding proteins	GP				NULL	In vitro	NULL	NULL	NULL	NULL	gw60_genesdev_11_17_2239_s_102	9303539	( A) In vitro binding of Eps15 to Gst fusions of EH-binding proteins.	bind
58034	1	500	5	NULL	NULL	0	NULL	Trn2	GP		is					transportin 2	GP				NULL		0	NULL	NULL	NULL	gw60_science_294_5548_1895_s_152	11729309	( A) In vitro binding of transportin 2 (Trn2)  to HuR is mediated by HNS.	bind
58035	2	500	5	NULL	NULL	0	NULL	Trn2	GP		bind					HuR	GP				NULL	in vitro	0	NULL	NULL	NULL	gw60_science_294_5548_1895_s_152	11729309	( A) In vitro binding of transportin 2 (Trn2)  to HuR is mediated by HNS.	bind
58036	3	500	5	NULL	NULL	0	NULL	statement 1	Process		is mediated by					HNS	GP				NULL	in vitro	0	NULL	NULL	NULL	gw60_science_294_5548_1895_s_152	11729309	( A) In vitro binding of transportin 2 (Trn2)  to HuR is mediated by HNS.	bind
1620	1	500	6	NULL	NULL	0	NULL	Trn2	GP		bind					HuR	GP				NULL	In vitro	NULL	NULL	NULL	NULL	gw60_science_294_5548_1895_s_152	11729309	( A) In vitro binding of transportin 2 (Trn2)  to HuR is mediated by HNS.	bind
1621	2	500	6	NULL	NULL	0	NULL	HNS	AminoAcid		mediates					Statement 1					NULL		NULL	NULL	NULL	NULL	gw60_science_294_5548_1895_s_152	11729309	( A) In vitro binding of transportin 2 (Trn2)  to HuR is mediated by HNS.	bind
51786	3	500	6	10	NULL	0	NULL	Trn2	NULL		is	NULL				transportin 2	NULL				NULL		0	NULL	NULL	NULL	gw60_science_294_5548_1895_s_152	11729309	( A) In vitro binding of transportin 2 (Trn2)  to HuR is mediated by HNS.	bind
58037	1	503	5	NULL	NULL	0	NULL	GRIP1	GP		bind			NID		TRbeta	GP		LBD		NULL		0	NULL	NULL	NULL	gw60_genesdev_12_21_3343_s_139	9808622	( a) Individual leucine residues of the LxxLL motif are crucial for binding of GRIP1 NID to TRbeta LBD.	bind
58038	2	503	5	NULL	NULL	0	NULL				is crucial for			leucine residues of the LxxLL motif		statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_21_3343_s_139	9808622	( a) Individual leucine residues of the LxxLL motif are crucial for binding of GRIP1 NID to TRbeta LBD.	bind
1622	1	503	6	NULL	NULL	0	NULL	GRIP1	GP		bind			NID		TRbeta	GP		LBD		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_21_3343_s_139	9808622	( a) Individual leucine residues of the LxxLL motif are crucial for binding of GRIP1 NID to TRbeta LBD.	bind
1623	2	503	6	NULL	NULL	0	NULL	 	AminoAcid		are crucial for			leucine residues of the LxxLL motif		Statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_21_3343_s_139	9808622	( a) Individual leucine residues of the LxxLL motif are crucial for binding of GRIP1 NID to TRbeta LBD.	bind
58039	1	507	5	NULL	NULL	0	NULL	Mlc	GP		bind					target DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_embo_20_3_491_s_131	11157755	( A) Inhibition of Mlc binding to its target DNA by dephosphorylated EIICBGlc.	bind
58040	2	507	5	NULL	NULL	0	NULL	EIICBGlc	GP	dephosphorylated	inhibits					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_embo_20_3_491_s_131	11157755	( A) Inhibition of Mlc binding to its target DNA by dephosphorylated EIICBGlc.	bind
1624	1	507	6	NULL	NULL	0	NULL	Mlc	GP		bind					target DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_491_s_131	11157755	( A) Inhibition of Mlc binding to its target DNA by dephosphorylated EIICBGlc.	bind
1625	2	507	6	NULL	NULL	0	NULL	EIICBGlc	GP	dephosphorylated	inhibits					Statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_491_s_131	11157755	( A) Inhibition of Mlc binding to its target DNA by dephosphorylated EIICBGlc.	bind
58041	1	508	5	NULL	NULL	0	NULL	STAT5	GP		bind					DNA	NucleicAcid				NULL	transfected D10 clone	NULL	NULL	NULL	NULL	gw60_science_283_5399_222_s_145	9880255	( A) Inhibition of STAT5-DNA binding by  FLAG STAT5 Y694F in a transfected D10 clone.	bind
58042	2	508	5	NULL	NULL	0	NULL	STAT5	GP	FLAG-tagged	inhibits			Y694F		statement 1	Process				NULL	transfected D10 clone	0	NULL	NULL	NULL	gw60_science_283_5399_222_s_145	9880255	( A) Inhibition of STAT5-DNA binding by  FLAG STAT5 Y694F in a transfected D10 clone.	bind
1626	1	508	6	NULL	NULL	0	NULL	STAT5	GP		bind					DNA	NucleicAcid				NULL	transfected D10 clone	NULL	NULL	NULL	NULL	gw60_science_283_5399_222_s_145	9880255	( A) Inhibition of STAT5-DNA binding by  FLAG STAT5 Y694F in a transfected D10 clone.	bind
1627	2	508	6	NULL	NULL	0	NULL	STAT5	GP		inhibit			y694F		statement1	Process				NULL	transfected D10 clone	NULL	NULL	NULL	NULL	gw60_science_283_5399_222_s_145	9880255	( A) Inhibition of STAT5-DNA binding by  FLAG STAT5 Y694F in a transfected D10 clone.	bind
58043	1	510	5	NULL	NULL	0	NULL	IpaA	GP		bind					vinculin	GP				NULL		0	NULL	NULL	NULL	gw60_embo_18_21_5853_s_292	10545097	( A) IpaA binds to vinculin and leads to a conformational change of vinculin (arrow 1).	bind
58044	2	510	5	NULL	NULL	0	NULL	statement 1	Process		changes					vinculin	GP	conformation of			NULL		0	NULL	NULL	NULL	gw60_embo_18_21_5853_s_292	10545097	( A) IpaA binds to vinculin and leads to a conformational change of vinculin (arrow 1).	bind
1628	1	510	6	NULL	NULL	0	NULL	IpaA	GP		bind					vinculin	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_5853_s_292	10545097	( A) IpaA binds to vinculin and leads to a conformational change of vinculin (arrow 1).	bind
1629	2	510	6	NULL	NULL	0	NULL	Statement 1	Process		leads to					vinculin	GP	conformational change of			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_5853_s_292	10545097	( A) IpaA binds to vinculin and leads to a conformational change of vinculin (arrow 1).	bind
58045	1	511	5	NULL	NULL	0	NULL				does not bind			K145E ( spt15-640)		Mot1	GP				NULL		0	NULL	NULL	NULL	gw60_embo_18_23_6662_s_158	10581240	( A) K145E ( spt15-640) fails to bind Mot1.	bind
1630	1	511	6	NULL	NULL	0	NULL		AminoAcid		fails to bind			K145E ( spt15-640)		Mot1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_23_6662_s_158	10581240	( A) K145E ( spt15-640) fails to bind Mot1.	bind
58046	1	512	5	NULL	NULL	0	NULL	GST-PDZ1	GP		bind					CFTR	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_98_3_1300_s_137	11158634	( A) Kinetic-response data for GST-PDZ1 binding to CFTR.	bind
1631	1	512	6	NULL	NULL	0	NULL	GST-PDZ1	GP		bind					CFTR	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_3_1300_s_137	11158634	( A) Kinetic-response data for GST-PDZ1 binding to CFTR.	bind
58047	1	513	5	NULL	NULL	0	NULL	NCp	GP		bind					T-ODN1	GP				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_31_19_5754_s_85	14500839	( A) Kinetics of NCp binding to T-ODN1 with no added constituents.	bind
1632	1	513	6	NULL	NULL	0	NULL	NCp	GP		bind					T-ODN1	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_19_5754_s_85	14500839	( A) Kinetics of NCp binding to T-ODN1 with no added constituents.	bind
58048	1	514	5	NULL	NULL	0	NULL	PTH	GP		bind			(1-34)TMR		GFPN-PTHR	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_102_44_16084_s_123	16236727	( A) Kinetics of PTH(1-34)TMR binding to GFPN-PTHR recorded by decreases in the fluorescence emission of the GFP moiety.	bind
1633	1	514	6	NULL	NULL	0	NULL	PTH-TMR	GP		bind			1-34		GFPN-PTHR	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_44_16084_s_123	16236727	( A) Kinetics of PTH(1-34)TMR binding to GFPN-PTHR recorded by decreases in the fluorescence emission of the GFP moiety.	bind
58049	1	515	5	NULL	NULL	0	NULL	Ste5	GP		bind					Ste4	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_13_2564_s_108	15192700	( A) Kss1 activation is dependent on Ste5 binding to Ste4 and Ste11.	bind
58050	2	515	5	NULL	NULL	0	NULL	Ste5	GP		bind					Ste11	GP				NULL		0	NULL	NULL	NULL	gw70_embo_23_13_2564_s_108	15192700	( A) Kss1 activation is dependent on Ste5 binding to Ste4 and Ste11.	bind
58051	3	515	5	NULL	NULL	0	NULL	Kss1	GP	activation of	is dependent on					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_embo_23_13_2564_s_108	15192700	( A) Kss1 activation is dependent on Ste5 binding to Ste4 and Ste11.	bind
58052	4	515	5	NULL	NULL	0	NULL	Kss1	GP	activation of	is dependent on					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_embo_23_13_2564_s_108	15192700	( A) Kss1 activation is dependent on Ste5 binding to Ste4 and Ste11.	bind
1634	1	515	6	NULL	NULL	0	NULL	Ste5	GP		bind					Ste4	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_13_2564_s_108	15192700	( A) Kss1 activation is dependent on Ste5 binding to Ste4 and Ste11.	bind
1635	2	515	6	NULL	NULL	0	NULL	Ste5	GP		bind					Ste11	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_13_2564_s_108	15192700	( A) Kss1 activation is dependent on Ste5 binding to Ste4 and Ste11.	bind
1637	3	515	6	NULL	NULL	0	NULL	Kss1	GP	activation of	is dependent on					Statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_13_2564_s_108	15192700	( A) Kss1 activation is dependent on Ste5 binding to Ste4 and Ste11.	bind
58053	1	517	5	NULL	NULL	0	NULL	Lef-1	GP		bind					siamois	GP			promoter	NULL		0	NULL	NULL	NULL	gw60_genesdev_11_18_2359_s_119	9308964	( A) Lef-1 binding to the  siamois promoter is competed by an oligonucleotide containing a consensus Lef/Tcf-binding site.	bind
58054	2	517	5	NULL	NULL	0	NULL	oligonucleotide	NucleicAcid		contains							consensus		Lef/Tcf-binding site	NULL		0	NULL	NULL	NULL	gw60_genesdev_11_18_2359_s_119	9308964	( A) Lef-1 binding to the  siamois promoter is competed by an oligonucleotide containing a consensus Lef/Tcf-binding site.	bind
58055	3	517	5	NULL	NULL	0	NULL	statement 2	NucleicAcid		bind					siamois	GP			promoter	NULL		0	NULL	NULL	NULL	gw60_genesdev_11_18_2359_s_119	9308964	( A) Lef-1 binding to the  siamois promoter is competed by an oligonucleotide containing a consensus Lef/Tcf-binding site.	bind
58056	4	517	5	NULL	NULL	0	NULL	statement 3	Process		competes with					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_genesdev_11_18_2359_s_119	9308964	( A) Lef-1 binding to the  siamois promoter is competed by an oligonucleotide containing a consensus Lef/Tcf-binding site.	bind
1638	1	517	6	NULL	NULL	0	NULL	Lef-1	GP		bind					Siamois	GP			Promoter	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_18_2359_s_119	9308964	( A) Lef-1 binding to the  siamois promoter is competed by an oligonucleotide containing a consensus Lef/Tcf-binding site.	bind
1639	2	517	6	NULL	NULL	0	NULL	oligonucleotide	NucleicAcid		bind				consensus Lef/Tcf-binding site	Siamois	GP			Promoter	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_18_2359_s_119	9308964	( A) Lef-1 binding to the  siamois promoter is competed by an oligonucleotide containing a consensus Lef/Tcf-binding site.	bind
51787	3	517	6	NULL	NULL	0	NULL	statement 1	Process		compete with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_18_2359_s_119	9308964	( A) Lef-1 binding to the  siamois promoter is competed by an oligonucleotide containing a consensus Lef/Tcf-binding site.	bind
58057	1	520	5	NULL	NULL	0	NULL	LPS	GP		bind					Hsp 90	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_96_10_5645_s_131	10318938	( A) LPS binds Hsp 90 but not ovalbumin.	bind
58058	2	520	5	NULL	NULL	0	NULL	LPS	GP		does not bind					ovalbumin	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_96_10_5645_s_131	10318938	( A) LPS binds Hsp 90 but not ovalbumin.	bind
1640	1	520	6	NULL	NULL	0	NULL	LPS	Chemical		bind					Hsp 90	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_10_5645_s_131	10318938	( A) LPS binds Hsp 90 but not ovalbumin.	bind
1641	2	520	6	NULL	NULL	0	NULL	LPS	Chemical		does not bind					ovalbumin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_10_5645_s_131	10318938	( A) LPS binds Hsp 90 but not ovalbumin.	bind
58059	1	523	5	NULL	NULL	0	NULL	mbeta2M	GP	wt	does not bind					ThT	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_29_10584_s_55	15249659	( A) mbeta2M/wt (filled circles) does not bind ThT.	bind
1642	1	523	6	NULL	NULL	0	NULL	mbeta2M	GP	wild type	does not bind					ThT	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_29_10584_s_55	15249659	( A) mbeta2M/wt (filled circles) does not bind ThT.	bind
58060	1	524	5	NULL	NULL	0	NULL	MBP	GP		bind					maltose	Chemical				NULL		0	NULL	NULL	NULL	gw60_pnas_98_4_1525_s_130	11171984	( A) MBP binds maltose and undergoes a conformational change from an open to a closed conformation, generating a high-affinity sugar-binding site.	bind
58061	2	524	5	NULL	NULL	0	NULL	statement 1	Process		changes					MBP	GP	conformation of			NULL		0	NULL	NULL	NULL	gw60_pnas_98_4_1525_s_130	11171984	( A) MBP binds maltose and undergoes a conformational change from an open to a closed conformation, generating a high-affinity sugar-binding site.	bind
58062	3	524	5	NULL	NULL	0	NULL	statement 2	Process		generates							high-affinity	sugar-binding site		NULL		0	NULL	NULL	NULL	gw60_pnas_98_4_1525_s_130	11171984	( A) MBP binds maltose and undergoes a conformational change from an open to a closed conformation, generating a high-affinity sugar-binding site.	bind
1643	1	524	6	NULL	NULL	0	NULL	MBP	GP		bind					maltose	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_4_1525_s_130	11171984	( A) MBP binds maltose and undergoes a conformational change from an open to a closed conformation, generating a high-affinity sugar-binding site.	bind
1644	2	524	6	NULL	NULL	0	NULL	Statement 1	Process		change					MBP	GP	conformation of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_4_1525_s_130	11171984	( A) MBP binds maltose and undergoes a conformational change from an open to a closed conformation, generating a high-affinity sugar-binding site.	bind
1645	3	524	6	NULL	NULL	0	NULL	Statement 2	Process		generates						GP	high-affinity		sugar-binding site	NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_4_1525_s_130	11171984	( A) MBP binds maltose and undergoes a conformational change from an open to a closed conformation, generating a high-affinity sugar-binding site.	bind
58063	1	525	5	NULL	NULL	0	NULL	MECA-79	GP		bind					CHO-PSGL-1	Cell				NULL		0	NULL	NULL	NULL	gw70_pnas_101_51_17807_s_113	15591109	( A) MECA-79 binds CHO cells expressing 6-sulfo sialyl Lewis X on extended core 1 (CHO-PSGL-1.	bind
58064	2	525	5	NULL	NULL	0	NULL	CHO-PSGL-1	Cell		is					CHO cells expressing 6-sulfo sialyl Lewis X on extended core 1 	Cell				NULL		0	NULL	NULL	NULL	gw70_pnas_101_51_17807_s_113	15591109	( A) MECA-79 binds CHO cells expressing 6-sulfo sialyl Lewis X on extended core 1 (CHO-PSGL-1.	bind
1636	1	525	6	NULL	NULL	0	NULL	MECA-79	GP		bind					PSGL-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_51_17807_s_113	15591109	( A) MECA-79 binds CHO cells expressing 6-sulfo sialyl Lewis X on extended core 1 (CHO-PSGL-1.	bind
2221	2	525	6	NULL	NULL	0	NULL	PSGL-1	GP		is expressed on					CHO cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_51_17807_s_113	15591109	( A) MECA-79 binds CHO cells expressing 6-sulfo sialyl Lewis X on extended core 1 (CHO-PSGL-1.	bind
58065	1	527	5	NULL	NULL	0	NULL	neutrophils	Cell	unstimulated;;human	bind					Fg	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_102_5_1614_s_83	15665082	( A) Micrographs of wells with unstimulated ( Left) or TNF-stimulated ( Center) human neutrophils binding to Fg, or unstimulated neutrophils binding to plasmin-treated  Fg ( Right).	bind
58066	2	527	5	NULL	NULL	0	NULL	neutrophils	Cell	human	is stimulated by					TNF	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_102_5_1614_s_83	15665082	( A) Micrographs of wells with unstimulated ( Left) or TNF-stimulated ( Center) human neutrophils binding to Fg, or unstimulated neutrophils binding to plasmin-treated  Fg ( Right).	bind
58067	3	527	5	NULL	NULL	0	NULL	statement 2	Cell		bind					Fg	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1614_s_83	15665082	( A) Micrographs of wells with unstimulated ( Left) or TNF-stimulated ( Center) human neutrophils binding to Fg, or unstimulated neutrophils binding to plasmin-treated  Fg ( Right).	bind
58068	4	527	5	NULL	NULL	0	NULL	neutrophils	Cell	unstimulated	bind					Fg	GP	plasmin-treated			NULL		0	NULL	NULL	NULL	gw70_pnas_102_5_1614_s_83	15665082	( A) Micrographs of wells with unstimulated ( Left) or TNF-stimulated ( Center) human neutrophils binding to Fg, or unstimulated neutrophils binding to plasmin-treated  Fg ( Right).	bind
1646	1	527	6	NULL	NULL	0	NULL	neutrophils	Cell	human;;unstimulated	bind					Fg	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1614_s_83	15665082	( A) Micrographs of wells with unstimulated ( Left) or TNF-stimulated ( Center) human neutrophils binding to Fg, or unstimulated neutrophils binding to plasmin-treated  Fg ( Right).	bind
1647	3	527	6	NULL	NULL	0	NULL	statement 2	Process		bind					Fg	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1614_s_83	15665082	( A) Micrographs of wells with unstimulated ( Left) or TNF-stimulated ( Center) human neutrophils binding to Fg, or unstimulated neutrophils binding to plasmin-treated  Fg ( Right).	bind
1648	4	527	6	NULL	NULL	0	NULL	neutrophils	Cell	human;;unstimulated	bind					Fg	GP	plasmin-treated			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1614_s_83	15665082	( A) Micrographs of wells with unstimulated ( Left) or TNF-stimulated ( Center) human neutrophils binding to Fg, or unstimulated neutrophils binding to plasmin-treated  Fg ( Right).	bind
51831	2	527	6	NULL	NULL	0	NULL	TNF	GP		stimulate					neutrophils	Cell	human			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1614_s_83	15665082	( A) Micrographs of wells with unstimulated ( Left) or TNF-stimulated ( Center) human neutrophils binding to Fg, or unstimulated neutrophils binding to plasmin-treated  Fg ( Right).	bind
58069	1	528	5	NULL	NULL	0	NULL	MLL-AF4	GP		bind					CDKN1B	GP			promoter	NULL		0	NULL	NULL	NULL	gw70_pnas_102_39_14028_s_221	16169901	( A) MLL-AF4 binds to the  CDKN1B promoter ( Left) but not to the  CDKN1B coding region	bind
58070	2	528	5	NULL	NULL	0	NULL	MLL-AF4	GP		does not bind					CDKN1B	GP			coding region	NULL		0	NULL	NULL	NULL	gw70_pnas_102_39_14028_s_221	16169901	( A) MLL-AF4 binds to the  CDKN1B promoter ( Left) but not to the  CDKN1B coding region	bind
1649	1	528	6	NULL	NULL	0	NULL	MLL-AF4	GP		bind					CDKN1B	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_39_14028_s_221	16169901	( A) MLL-AF4 binds to the  CDKN1B promoter ( Left) but not to the  CDKN1B coding region	bind
1650	2	528	6	NULL	NULL	0	NULL	MLL-AF4	GP		does not bind					CDKN1B	GP		coding region		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_39_14028_s_221	16169901	( A) MLL-AF4 binds to the  CDKN1B promoter ( Left) but not to the  CDKN1B coding region	bind
58071	1	531	5	NULL	NULL	0	NULL	ERM proteins	GP		bind					PIP2	GP				NULL	membrane	0	NULL	NULL	NULL	gw70_embo_22_3_502_s_188	12554651	( A) Model of ERM proteins bound to both PIP2 in a membrane and the ICAM-2 cytoplasmic  tail.	bind
58072	2	531	5	NULL	NULL	0	NULL	ERM proteins	GP		bind					ICAM-2	GP		cytoplasmic tail		NULL		0	NULL	NULL	NULL	gw70_embo_22_3_502_s_188	12554651	( A) Model of ERM proteins bound to both PIP2 in a membrane and the ICAM-2 cytoplasmic  tail.	bind
1651	1	531	6	NULL	NULL	0	NULL	ERM protein	GP		bind					PIP2	GP				NULL	membrane	NULL	NULL	NULL	NULL	gw70_embo_22_3_502_s_188	12554651	( A) Model of ERM proteins bound to both PIP2 in a membrane and the ICAM-2 cytoplasmic  tail.	bind
1652	2	531	6	NULL	NULL	0	NULL	ERM protein	GP		bind					ICAM-2	GP		cytoplasmic tail		NULL		NULL	NULL	NULL	NULL	gw70_embo_22_3_502_s_188	12554651	( A) Model of ERM proteins bound to both PIP2 in a membrane and the ICAM-2 cytoplasmic  tail.	bind
58073	1	534	5	NULL	NULL	0	NULL	LdTOP1	GP	putative	bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_3_794_s_169	11809893	( A) Model of the inhibitor CPT bound to the covalent complex of putative LdTOP1 and DNA.	bind
58074	2	534	5	NULL	NULL	0	NULL	statement 1	Process		forms					covalent complex					NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_3_794_s_169	11809893	( A) Model of the inhibitor CPT bound to the covalent complex of putative LdTOP1 and DNA.	bind
58075	3	534	5	NULL	NULL	0	NULL	CPT	Chemical		is a type of					inhibitor					NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_3_794_s_169	11809893	( A) Model of the inhibitor CPT bound to the covalent complex of putative LdTOP1 and DNA.	bind
58076	4	534	5	NULL	NULL	0	NULL	CPT	Chemical		bind					statement 1	GP				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_3_794_s_169	11809893	( A) Model of the inhibitor CPT bound to the covalent complex of putative LdTOP1 and DNA.	bind
1653	1	534	6	NULL	NULL	0	NULL	LdTOP1	GP	putative	bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_3_794_s_169	11809893	( A) Model of the inhibitor CPT bound to the covalent complex of putative LdTOP1 and DNA.	bind
1654	2	534	6	NULL	NULL	0	NULL	Statement 1	Process		forms a					covalent complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_3_794_s_169	11809893	( A) Model of the inhibitor CPT bound to the covalent complex of putative LdTOP1 and DNA.	bind
1655	3	534	6	NULL	NULL	0	NULL	CPT	Chemical	inhibitor	bind					Statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_3_794_s_169	11809893	( A) Model of the inhibitor CPT bound to the covalent complex of putative LdTOP1 and DNA.	bind
58077	1	535	5	NULL	NULL	0	NULL	LFA-1	GP		bind					ICAM-1 dimers	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_98_12_6830_s_43	11391003	( A) Models of LFA-1 binding to ICAM-1 dimers.	bind
1656	1	535	6	NULL	NULL	0	NULL	LFA-1	GP		bind					ICAM-1 dimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_12_6830_s_43	11391003	( A) Models of LFA-1 binding to ICAM-1 dimers.	bind
58078	1	537	5	NULL	NULL	0	NULL	MT	CellComponent		bind					EGFP-NCFC	GP	wild type			NULL		0	NULL	NULL	NULL	gw70_embo_23_7_1506_s_156	15014437	( A) MT binding of EGFP-NCFC (wild type and Y649F) and MCFC-EGFP (wild type and Y649F).	bind
58079	2	537	5	NULL	NULL	0	NULL	MT	CellComponent		bind					EGFP-NCFC	GP		Y649F		NULL		0	NULL	NULL	NULL	gw70_embo_23_7_1506_s_156	15014437	( A) MT binding of EGFP-NCFC (wild type and Y649F) and MCFC-EGFP (wild type and Y649F).	bind
58080	3	537	5	NULL	NULL	0	NULL	MT	CellComponent		bind					MCFC-EGFP	GP	wild type			NULL		0	NULL	NULL	NULL	gw70_embo_23_7_1506_s_156	15014437	( A) MT binding of EGFP-NCFC (wild type and Y649F) and MCFC-EGFP (wild type and Y649F).	bind
58081	4	537	5	NULL	NULL	0	NULL	MT	CellComponent		bind					MCFC-EGFP	GP		Y649F		NULL		0	NULL	NULL	NULL	gw70_embo_23_7_1506_s_156	15014437	( A) MT binding of EGFP-NCFC (wild type and Y649F) and MCFC-EGFP (wild type and Y649F).	bind
1657	1	537	6	NULL	NULL	0	NULL	MT	CellComponent		bind					 EGFP-NCFC	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1506_s_156	15014437	( A) MT binding of EGFP-NCFC (wild type and Y649F) and MCFC-EGFP (wild type and Y649F).	bind
1658	2	537	6	10	NULL	0	NULL	MT	NULL		bind	NULL				MCFC-EGFP	NULL	wild type			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1506_s_156	15014437	( A) MT binding of EGFP-NCFC (wild type and Y649F) and MCFC-EGFP (wild type and Y649F).	bind
51833	3	537	6	10	NULL	0	NULL	MT	NULL		bind	NULL				EGFP-NCFC	NULL		Y649F		NULL		0	NULL	NULL	NULL	gw70_embo_23_7_1506_s_156	15014437	( A) MT binding of EGFP-NCFC (wild type and Y649F) and MCFC-EGFP (wild type and Y649F).	bind
51834	4	537	6	10	NULL	0	NULL	MT	NULL		bind	NULL				MCFC-EGFP	NULL		Y649F		NULL		0	NULL	NULL	NULL	gw70_embo_23_7_1506_s_156	15014437	( A) MT binding of EGFP-NCFC (wild type and Y649F) and MCFC-EGFP (wild type and Y649F).	bind
58082	1	538	5	NULL	NULL	0	NULL	SIP1 polypeptide	GP		bind			NZF		DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5073_s_191	10487759	( A) Mutations within NZF3, NZF4, CZF2 and CZF3 abolish DNA binding of short SIP1NZF and SIP1CZF polypeptides.	bind
58083	2	538	5	NULL	NULL	0	NULL	SIP1 polypeptide	GP		bind			CZF		DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5073_s_191	10487759	( A) Mutations within NZF3, NZF4, CZF2 and CZF3 abolish DNA binding of short SIP1NZF and SIP1CZF polypeptides.	bind
58084	3	538	5	NULL	NULL	0	NULL	NZF3	GP	mutant	abolishes					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_18_5073_s_191	10487759	( A) Mutations within NZF3, NZF4, CZF2 and CZF3 abolish DNA binding of short SIP1NZF and SIP1CZF polypeptides.	bind
58085	4	538	5	NULL	NULL	0	NULL	NZF3	GP	mutant	abolishes					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_18_5073_s_191	10487759	( A) Mutations within NZF3, NZF4, CZF2 and CZF3 abolish DNA binding of short SIP1NZF and SIP1CZF polypeptides.	bind
58086	5	538	5	NULL	NULL	0	NULL	NZF4	GP	mutant	abolishes					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_18_5073_s_191	10487759	( A) Mutations within NZF3, NZF4, CZF2 and CZF3 abolish DNA binding of short SIP1NZF and SIP1CZF polypeptides.	bind
58087	6	538	5	NULL	NULL	0	NULL	NZF4	GP	mutant	abolishes					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_18_5073_s_191	10487759	( A) Mutations within NZF3, NZF4, CZF2 and CZF3 abolish DNA binding of short SIP1NZF and SIP1CZF polypeptides.	bind
58088	7	538	5	NULL	NULL	0	NULL	CZF2	GP	mutant	abolishes					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_18_5073_s_191	10487759	( A) Mutations within NZF3, NZF4, CZF2 and CZF3 abolish DNA binding of short SIP1NZF and SIP1CZF polypeptides.	bind
58089	8	538	5	NULL	NULL	0	NULL	CZF2	GP	mutant	abolishes					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_18_5073_s_191	10487759	( A) Mutations within NZF3, NZF4, CZF2 and CZF3 abolish DNA binding of short SIP1NZF and SIP1CZF polypeptides.	bind
58090	9	538	5	NULL	NULL	0	NULL	CZF3	GP	mutant	abolishes					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_18_5073_s_191	10487759	( A) Mutations within NZF3, NZF4, CZF2 and CZF3 abolish DNA binding of short SIP1NZF and SIP1CZF polypeptides.	bind
58091	10	538	5	NULL	NULL	0	NULL	CZF3	GP	mutant	abolishes					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_18_5073_s_191	10487759	( A) Mutations within NZF3, NZF4, CZF2 and CZF3 abolish DNA binding of short SIP1NZF and SIP1CZF polypeptides.	bind
1659	1	538	6	NULL	NULL	0	NULL	short SIP1 polypeptide	GP		bind			NZF		DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5073_s_191	10487759	( A) Mutations within NZF3, NZF4, CZF2 and CZF3 abolish DNA binding of short SIP1NZF and SIP1CZF polypeptides.	bind
1660	2	538	6	NULL	NULL	0	NULL	short SIP1 polypeptide	GP	mutant	abolish 			 NZF3		DNA	NucleicAcid	binding of			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5073_s_191	10487759	( A) Mutations within NZF3, NZF4, CZF2 and CZF3 abolish DNA binding of short SIP1NZF and SIP1CZF polypeptides.	bind
1661	3	538	6	NULL	NULL	0	NULL	short SIP1 polypeptide	GP	mutant	abolish 			 NZF4		DNA	NucleicAcid	binding of			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5073_s_191	10487759	( A) Mutations within NZF3, NZF4, CZF2 and CZF3 abolish DNA binding of short SIP1NZF and SIP1CZF polypeptides.	bind
1662	4	538	6	NULL	NULL	0	NULL	short SIP1 polypeptide	GP		bind			CZF		DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5073_s_191	10487759	( A) Mutations within NZF3, NZF4, CZF2 and CZF3 abolish DNA binding of short SIP1NZF and SIP1CZF polypeptides.	bind
1663	5	538	6	NULL	NULL	0	NULL	short SIP1 polypeptide	GP	mutant	abolish 			 CZF2		DNA	NucleicAcid	binding of			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5073_s_191	10487759	( A) Mutations within NZF3, NZF4, CZF2 and CZF3 abolish DNA binding of short SIP1NZF and SIP1CZF polypeptides.	bind
1664	6	538	6	NULL	NULL	0	NULL	short SIP1 polypeptide	GP	mutant	abolish 			CZF3		DNA	NucleicAcid	binding of			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5073_s_191	10487759	( A) Mutations within NZF3, NZF4, CZF2 and CZF3 abolish DNA binding of short SIP1NZF and SIP1CZF polypeptides.	bind
58092	1	539	5	NULL	NULL	0	NULL	Myozenin	GP		bind					alpha-actinin-2	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_98_4_1595_s_151	11171996	( A) Myozenin binds to both alpha-actinin-2 and -3 but not to itself ( Left), whereas alpha-actinin-2 and -3 both bind to myozenin as well as to themselves ( Center and  Right).	bind
58093	2	539	5	NULL	NULL	0	NULL	Myozenin	GP		bind					alpha-actinin-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_4_1595_s_151	11171996	( A) Myozenin binds to both alpha-actinin-2 and -3 but not to itself ( Left), whereas alpha-actinin-2 and -3 both bind to myozenin as well as to themselves ( Center and  Right).	bind
58094	3	539	5	NULL	NULL	0	NULL	Myozenin	GP		does not bind					Myozenin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_4_1595_s_151	11171996	( A) Myozenin binds to both alpha-actinin-2 and -3 but not to itself ( Left), whereas alpha-actinin-2 and -3 both bind to myozenin as well as to themselves ( Center and  Right).	bind
58095	4	539	5	NULL	NULL	0	NULL	alpha-actinin-2	GP		bind					alpha-actinin-2	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_98_4_1595_s_151	11171996	( A) Myozenin binds to both alpha-actinin-2 and -3 but not to itself ( Left), whereas alpha-actinin-2 and -3 both bind to myozenin as well as to themselves ( Center and  Right).	bind
58096	5	539	5	NULL	NULL	0	NULL	alpha-actinin-3	GP		bind					alpha-actinin-3	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_98_4_1595_s_151	11171996	( A) Myozenin binds to both alpha-actinin-2 and -3 but not to itself ( Left), whereas alpha-actinin-2 and -3 both bind to myozenin as well as to themselves ( Center and  Right).	bind
1900	1	539	6	NULL	NULL	0	NULL	Myozenin	GP		bind					alpha-actinin-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_4_1595_s_151	11171996	( A) Myozenin binds to both alpha-actinin-2 and -3 but not to itself ( Left), whereas alpha-actinin-2 and -3 both bind to myozenin as well as to themselves ( Center and  Right).	bind
1901	2	539	6	NULL	NULL	0	NULL	Myozenin	GP		bind					alpha-actinin-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_4_1595_s_151	11171996	( A) Myozenin binds to both alpha-actinin-2 and -3 but not to itself ( Left), whereas alpha-actinin-2 and -3 both bind to myozenin as well as to themselves ( Center and  Right).	bind
1902	3	539	6	NULL	NULL	0	NULL	Myozenin	GP		does not bind					Myozenin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_4_1595_s_151	11171996	( A) Myozenin binds to both alpha-actinin-2 and -3 but not to itself ( Left), whereas alpha-actinin-2 and -3 both bind to myozenin as well as to themselves ( Center and  Right).	bind
1903	4	539	6	NULL	NULL	0	NULL	alpha-actinin-2 	GP		bind					alpha-actinin-2 	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_4_1595_s_151	11171996	( A) Myozenin binds to both alpha-actinin-2 and -3 but not to itself ( Left), whereas alpha-actinin-2 and -3 both bind to myozenin as well as to themselves ( Center and  Right).	bind
1904	5	539	6	NULL	NULL	0	NULL	alpha-actinin-3	GP		bind					alpha-actinin-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_4_1595_s_151	11171996	( A) Myozenin binds to both alpha-actinin-2 and -3 but not to itself ( Left), whereas alpha-actinin-2 and -3 both bind to myozenin as well as to themselves ( Center and  Right).	bind
58097	1	541	5	NULL	NULL	0	NULL	Sec1	GP	neuronal	bind					syntaxin	GP		Habc domain;;SNARE motif		NULL		NULL	NULL	NULL	NULL	gw60_embo_21_22_6114_s_230	12426383	( A) Neuronal Sec1 (blue) binds syntaxin (Habc domain grey, SNARE motif red) in a closed conformation ( Misura  et al., 2000).	bind
1665	1	541	6	NULL	NULL	0	NULL	Sec1	GP	neuronal	bind					syntaxin	GP		Habc domain		NULL		NULL	NULL	NULL	NULL	gw60_embo_21_22_6114_s_230	12426383	( A) Neuronal Sec1 (blue) binds syntaxin (Habc domain grey, SNARE motif red) in a closed conformation ( Misura  et al., 2000).	bind
1666	2	541	6	NULL	NULL	0	NULL	Sec1	GP	neuronal	bind					syntaxin	GP			SNARE motif	NULL		NULL	NULL	NULL	NULL	gw60_embo_21_22_6114_s_230	12426383	( A) Neuronal Sec1 (blue) binds syntaxin (Habc domain grey, SNARE motif red) in a closed conformation ( Misura  et al., 2000).	bind
58098	1	542	5	NULL	NULL	0	NULL	NF-kappaB1 p50 homodimers	GP		bind					HIV-1	Organism	latent		promoter	NULL		0	NULL	NULL	NULL	gw70_embo_25_1_139_s_216	16319923	( A) NF-kappaB1 p50 homodimers bound to the latent HIV-1 promoter recruit HDAC1, which deacetylates  regional histones and compacts local histone structure, thereby inhibiting the binding  of RNA Pol II.	bind
58099	2	542	5	NULL	NULL	0	NULL	statement 1	Process		recruit					HDAC1	GP				NULL		0	NULL	NULL	NULL	gw70_embo_25_1_139_s_216	16319923	( A) NF-kappaB1 p50 homodimers bound to the latent HIV-1 promoter recruit HDAC1, which deacetylates  regional histones and compacts local histone structure, thereby inhibiting the binding  of RNA Pol II.	bind
58100	3	542	5	NULL	NULL	0	NULL	HDAC1	GP		deacetylates					histones	GP	regional			NULL		0	NULL	NULL	NULL	gw70_embo_25_1_139_s_216	16319923	( A) NF-kappaB1 p50 homodimers bound to the latent HIV-1 promoter recruit HDAC1, which deacetylates  regional histones and compacts local histone structure, thereby inhibiting the binding  of RNA Pol II.	bind
58101	4	542	5	NULL	NULL	0	NULL	statement 3	Process		compacts					histone	GP	local  structure of			NULL		0	NULL	NULL	NULL	gw70_embo_25_1_139_s_216	16319923	( A) NF-kappaB1 p50 homodimers bound to the latent HIV-1 promoter recruit HDAC1, which deacetylates  regional histones and compacts local histone structure, thereby inhibiting the binding  of RNA Pol II.	bind
58102	5	542	5	NULL	NULL	0	NULL	statement 4	Process		inhibits					RNA Pol II	GP	binding of			NULL		0	NULL	NULL	NULL	gw70_embo_25_1_139_s_216	16319923	( A) NF-kappaB1 p50 homodimers bound to the latent HIV-1 promoter recruit HDAC1, which deacetylates  regional histones and compacts local histone structure, thereby inhibiting the binding  of RNA Pol II.	bind
1667	1	542	6	NULL	NULL	0	NULL	 NF-kappaB1 p50 homodimers	GP		bind					HIV-1	NucleicAcid	latent		Promoter	NULL		NULL	NULL	NULL	NULL	gw70_embo_25_1_139_s_216	16319923	( A) NF-kappaB1 p50 homodimers bound to the latent HIV-1 promoter recruit HDAC1, which deacetylates  regional histones and compacts local histone structure, thereby inhibiting the binding  of RNA Pol II.	bind
1668	2	542	6	NULL	NULL	0	NULL	 NF-kappaB1 p50 homodimers	GP		recruit					HDAC1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_1_139_s_216	16319923	( A) NF-kappaB1 p50 homodimers bound to the latent HIV-1 promoter recruit HDAC1, which deacetylates  regional histones and compacts local histone structure, thereby inhibiting the binding  of RNA Pol II.	bind
1669	3	542	6	NULL	NULL	0	NULL	HDAC1	GP		deacetylates					regional histones	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_1_139_s_216	16319923	( A) NF-kappaB1 p50 homodimers bound to the latent HIV-1 promoter recruit HDAC1, which deacetylates  regional histones and compacts local histone structure, thereby inhibiting the binding  of RNA Pol II.	bind
1670	4	542	6	NULL	NULL	0	NULL	HDAC1	GP		compacts					histone 	GP	local;; structure of			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_1_139_s_216	16319923	( A) NF-kappaB1 p50 homodimers bound to the latent HIV-1 promoter recruit HDAC1, which deacetylates  regional histones and compacts local histone structure, thereby inhibiting the binding  of RNA Pol II.	bind
1671	5	542	6	NULL	NULL	0	NULL	Statement 3	Process		inhibit					RNA Pol II	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_1_139_s_216	16319923	( A) NF-kappaB1 p50 homodimers bound to the latent HIV-1 promoter recruit HDAC1, which deacetylates  regional histones and compacts local histone structure, thereby inhibiting the binding  of RNA Pol II.	bind
1672	6	542	6	NULL	NULL	0	NULL	Statement 4	Process		inhibit					RNA Pol II	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_1_139_s_216	16319923	( A) NF-kappaB1 p50 homodimers bound to the latent HIV-1 promoter recruit HDAC1, which deacetylates  regional histones and compacts local histone structure, thereby inhibiting the binding  of RNA Pol II.	bind
58103	1	543	5	NULL	NULL	0	NULL	Raf-1	GP		bind					Rb	GP				NULL	HAEC cells	0	NULL	NULL	NULL	gw70_jclininvest_116_8_2208_s_80	16862215	( A) Nicotine induces the binding of Raf-1 to Rb in HAEC and A549 cells as seen by IP/Western  blotting.	bind
58104	2	543	5	NULL	NULL	0	NULL	Raf-1	GP		bind					Rb	GP				NULL	A549 cells	0	NULL	NULL	NULL	gw70_jclininvest_116_8_2208_s_80	16862215	( A) Nicotine induces the binding of Raf-1 to Rb in HAEC and A549 cells as seen by IP/Western  blotting.	bind
58105	3	543	5	NULL	NULL	0	NULL	Nicotine	Chemical		induce					statement 1	Process				NULL	HAEC cells	0	NULL	NULL	NULL	gw70_jclininvest_116_8_2208_s_80	16862215	( A) Nicotine induces the binding of Raf-1 to Rb in HAEC and A549 cells as seen by IP/Western  blotting.	bind
58106	4	543	5	NULL	NULL	0	NULL	Nicotine	Chemical		induce					statement 2	Process				NULL	A549 cells	0	NULL	NULL	NULL	gw70_jclininvest_116_8_2208_s_80	16862215	( A) Nicotine induces the binding of Raf-1 to Rb in HAEC and A549 cells as seen by IP/Western  blotting.	bind
1673	1	543	6	NULL	NULL	0	NULL	Raf-1	GP		bind					Rb	GP				NULL	HAEC cells	NULL	NULL	NULL	NULL	gw70_jclininvest_116_8_2208_s_80	16862215	( A) Nicotine induces the binding of Raf-1 to Rb in HAEC and A549 cells as seen by IP/Western  blotting.	bind
1674	2	543	6	NULL	NULL	0	NULL	Nicotine	Chemical		induces					statement1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_8_2208_s_80	16862215	( A) Nicotine induces the binding of Raf-1 to Rb in HAEC and A549 cells as seen by IP/Western  blotting.	bind
1675	3	543	6	NULL	NULL	0	NULL	Raf-1	GP		bind					Rb	GP				NULL	A549 cells	NULL	NULL	NULL	NULL	gw70_jclininvest_116_8_2208_s_80	16862215	( A) Nicotine induces the binding of Raf-1 to Rb in HAEC and A549 cells as seen by IP/Western  blotting.	bind
1676	4	543	6	NULL	NULL	0	NULL	Nicotine	Chemical		induces					Statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_8_2208_s_80	16862215	( A) Nicotine induces the binding of Raf-1 to Rb in HAEC and A549 cells as seen by IP/Western  blotting.	bind
58107	1	545	5	NULL	NULL	0	NULL	Rpp29	GP		bind					M1 RNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_16_5120_s_238	16155184	( A) Northwestern blot analysis of binding of Rpp29 to M1 RNA.	bind
1677	1	545	6	NULL	NULL	0	NULL	Rpp29	GP		bind					M1 RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_16_5120_s_238	16155184	( A) Northwestern blot analysis of binding of Rpp29 to M1 RNA.	bind
58108	1	546	5	NULL	NULL	0	NULL	NSF	GP		bind					syntaxin Q226R-containing complexes	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_98_25_14262_s_120	11762430	( a) NSF binds to syntaxin Q226R-containing complexes via alpha-SNAP.	bind
58109	2	546	5	NULL	NULL	0	NULL	statement 1	Process		via					alpha-SNAP	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_98_25_14262_s_120	11762430	( a) NSF binds to syntaxin Q226R-containing complexes via alpha-SNAP.	bind
1678	1	546	6	NULL	NULL	0	NULL	NSF	GP		bind					syntaxin 	GP		Q226R-containing complexes		NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_25_14262_s_120	11762430	( a) NSF binds to syntaxin Q226R-containing complexes via alpha-SNAP.	bind
1679	2	546	6	NULL	NULL	0	NULL	Statement 1	Process		occurs via					alpha-SNAP	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_25_14262_s_120	11762430	( a) NSF binds to syntaxin Q226R-containing complexes via alpha-SNAP.	bind
58110	1	549	5	NULL	NULL	0	NULL	Sp-1	GP		is a type of					nuclear proteins	GP				NULL		0	NULL	NULL	NULL	gw60_jclininvest_102_10_1850_s_151	9819371	( A) Nuclear proteins binding to the Egr/Sp binding site of  the M-CSF promoter are Sp-1 and Sp-3.	bind
58111	2	549	5	NULL	NULL	0	NULL	Sp-3	GP		is a type of					nuclear protein	GP				NULL		0	NULL	NULL	NULL	gw60_jclininvest_102_10_1850_s_151	9819371	( A) Nuclear proteins binding to the Egr/Sp binding site of  the M-CSF promoter are Sp-1 and Sp-3.	bind
58112	3	549	5	NULL	NULL	0	NULL	Sp-1	GP		bind					M-CSF	GP			Egr/Sp binding site of promoter	NULL		0	NULL	NULL	NULL	gw60_jclininvest_102_10_1850_s_151	9819371	( A) Nuclear proteins binding to the Egr/Sp binding site of  the M-CSF promoter are Sp-1 and Sp-3.	bind
58113	4	549	5	NULL	NULL	0	NULL	Sp-3	GP		bind					M-CSF	GP			Egr/Sp binding site of promoter	NULL		0	NULL	NULL	NULL	gw60_jclininvest_102_10_1850_s_151	9819371	( A) Nuclear proteins binding to the Egr/Sp binding site of  the M-CSF promoter are Sp-1 and Sp-3.	bind
1682	1	549	6	NULL	NULL	0	NULL	Sp1	GP		bind					M-CSF	GP			Egr/Sp binding site in the promoter	NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_10_1850_s_151	9819371	( A) Nuclear proteins binding to the Egr/Sp binding site of  the M-CSF promoter are Sp-1 and Sp-3.	bind
1683	2	549	6	NULL	NULL	0	NULL	Sp-3	GP		bind					M-CSF	GP			Egr/Sp binding site in the promoter	NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_10_1850_s_151	9819371	( A) Nuclear proteins binding to the Egr/Sp binding site of  the M-CSF promoter are Sp-1 and Sp-3.	bind
58114	1	553	5	NULL	NULL	0	NULL	MR3.2scTCR 	GP	human	bind					MHC class II molecule	GP	rat			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_33_30961_s_178	12773544	( A) or  human MR3.2scTCR ( B) binding to a rat MHC class II molecule with  covalent Gp-BP-(69 - 89) (RTL201).	bind
1759	1	553	6	NULL	NULL	0	NULL	MR3.2scTCR	GP	human	bind			Gp-BP-(69 - 89) (RTL201)		MHC class II molecule	GP	rat			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_33_30961_s_178	12773544	( A) or  human MR3.2scTCR ( B) binding to a rat MHC class II molecule with  covalent Gp-BP-(69 - 89) (RTL201).	bind
58115	1	569	5	NULL	NULL	0	NULL	CR2	GP		bind					C3d	GP				NULL		0	NULL	NULL	NULL	gw60_science_292_5522_1725_s_34	11387479	( A) Overall view of the structure of CR2 binding to C3d.	bind
1760	1	569	6	NULL	NULL	0	NULL	CR2	GP		bind					C3d	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_292_5522_1725_s_34	11387479	( A) Overall view of the structure of CR2 binding to C3d.	bind
58116	1	573	5	NULL	NULL	0	NULL	p16	GP		bind					pRNA probe	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_21_4264_s_211	11691914	( A) p16 binds the pRNA probe with a  Kd = 1.5 x 10 - 7 (squares) an affinity 10-fold higher than that for the non-specific RNA240,  Kd  10 - 6 (circles).	bind
58117	2	573	5	NULL	NULL	0	NULL	p16	GP		bind					RNA240	NucleicAcid	non-specific			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_21_4264_s_211	11691914	( A) p16 binds the pRNA probe with a  Kd = 1.5 x 10 - 7 (squares) an affinity 10-fold higher than that for the non-specific RNA240,  Kd  10 - 6 (circles).	bind
58118	3	573	5	NULL	NULL	0	NULL	statement 1	Process	affinity of	is higher than					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_21_4264_s_211	11691914	( A) p16 binds the pRNA probe with a  Kd = 1.5 x 10 - 7 (squares) an affinity 10-fold higher than that for the non-specific RNA240,  Kd  10 - 6 (circles).	bind
1761	1	573	6	NULL	NULL	0	NULL	p16	GP		bind		high affinity			pRNA probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_21_4264_s_211	11691914	( A) p16 binds the pRNA probe with a  Kd = 1.5 x 10 - 7 (squares) an affinity 10-fold higher than that for the non-specific RNA240,  Kd  10 - 6 (circles).	bind
1762	2	573	6	NULL	NULL	0	NULL	p16	GP		bind		less affinity			RNA240	NucleicAcid	non-specific			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_21_4264_s_211	11691914	( A) p16 binds the pRNA probe with a  Kd = 1.5 x 10 - 7 (squares) an affinity 10-fold higher than that for the non-specific RNA240,  Kd  10 - 6 (circles).	bind
58119	1	574	5	NULL	NULL	0	NULL	p42	GP		bind					ErbB3 receptor	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_103_29_10917_s_181	16832058	( A) p42 but not p48 binds ErbB3 receptor.	bind
58120	2	574	5	NULL	NULL	0	NULL	p48	GP		does not bind					ErbB3 receptor	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_103_29_10917_s_181	16832058	( A) p42 but not p48 binds ErbB3 receptor.	bind
1763	1	574	6	NULL	NULL	0	NULL	p42	GP		bind					ErbB3 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_29_10917_s_181	16832058	( A) p42 but not p48 binds ErbB3 receptor.	bind
1764	2	574	6	NULL	NULL	0	NULL	p48	GP		does not bind					ErbB3 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_29_10917_s_181	16832058	( A) p42 but not p48 binds ErbB3 receptor.	bind
58121	1	575	5	NULL	NULL	0	NULL	p53 core	GP		bind					Hsp90	GP	native			NULL		0	NULL	NULL	NULL	gw60_pnas_99_17_11085_s_177	12163643	( A) p53 core binds Hsp90 in the native state.	bind
1765	1	575	6	NULL	NULL	0	NULL	p53	GP	core	bind					Hsp90	GP	native			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_17_11085_s_177	12163643	( A) p53 core binds Hsp90 in the native state.	bind
58122	1	576	5	NULL	NULL	0	NULL	p53	GP		recognizes					dsDNA oligonucleotides	NucleicAcid	internal gaps in			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_20_4005_s_65	11024181	( A) p53 recognises internal gaps in dsDNA oligonucleotides as short as 1 nt. Aliquots of 1 and 10 ng of unlabelled dsDNA oligonucleotides with internal single-strand gaps efficiently competed for p53 binding to the labelled ssDNA oligonucleotide NGC.	bind
58123	2	576	5	NULL	NULL	0	NULL	p53	GP		bind					ssDNA oligonucleotide NGC	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_20_4005_s_65	11024181	( A) p53 recognises internal gaps in dsDNA oligonucleotides as short as 1 nt. Aliquots of 1 and 10 ng of unlabelled dsDNA oligonucleotides with internal single-strand gaps efficiently competed for p53 binding to the labelled ssDNA oligonucleotide NGC.	bind
58124	3	576	5	NULL	NULL	0	NULL	dsDNA oligonucleotides	NucleicAcid	unlabeled	contains					single-strand gaps	NucleicAcid	internal			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_20_4005_s_65	11024181	( A) p53 recognises internal gaps in dsDNA oligonucleotides as short as 1 nt. Aliquots of 1 and 10 ng of unlabelled dsDNA oligonucleotides with internal single-strand gaps efficiently competed for p53 binding to the labelled ssDNA oligonucleotide NGC.	bind
58125	4	576	5	NULL	NULL	0	NULL	p53	GP		bind					statement 3	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_20_4005_s_65	11024181	( A) p53 recognises internal gaps in dsDNA oligonucleotides as short as 1 nt. Aliquots of 1 and 10 ng of unlabelled dsDNA oligonucleotides with internal single-strand gaps efficiently competed for p53 binding to the labelled ssDNA oligonucleotide NGC.	bind
58126	5	576	5	NULL	NULL	0	NULL	statement 4	Process		competes with		efficiently			statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_20_4005_s_65	11024181	( A) p53 recognises internal gaps in dsDNA oligonucleotides as short as 1 nt. Aliquots of 1 and 10 ng of unlabelled dsDNA oligonucleotides with internal single-strand gaps efficiently competed for p53 binding to the labelled ssDNA oligonucleotide NGC.	bind
1907	1	576	6	NULL	NULL	0	NULL	p53	GP		bind					ssDNA oligonucleotide NGC	NucleicAcid	labelled			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_20_4005_s_65	11024181	( A) p53 recognises internal gaps in dsDNA oligonucleotides as short as 1 nt. Aliquots of 1 and 10 ng of unlabelled dsDNA oligonucleotides with internal single-strand gaps efficiently competed for p53 binding to the labelled ssDNA oligonucleotide NGC.	bind
1908	2	576	6	NULL	NULL	0	NULL	p53	GP		bind					dsDNA oligonucleotides	NucleicAcid	unlabelled		internal single-strand gaps	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_20_4005_s_65	11024181	( A) p53 recognises internal gaps in dsDNA oligonucleotides as short as 1 nt. Aliquots of 1 and 10 ng of unlabelled dsDNA oligonucleotides with internal single-strand gaps efficiently competed for p53 binding to the labelled ssDNA oligonucleotide NGC.	bind
1909	3	576	6	NULL	NULL	0	NULL	p53	GP		recognizes					dsDNA oligonucleotide	NucleicAcid	internal gaps			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_20_4005_s_65	11024181	( A) p53 recognises internal gaps in dsDNA oligonucleotides as short as 1 nt. Aliquots of 1 and 10 ng of unlabelled dsDNA oligonucleotides with internal single-strand gaps efficiently competed for p53 binding to the labelled ssDNA oligonucleotide NGC.	bind
51835	4	576	6	NULL	NULL	0	NULL	statement 1	Process		compete with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_20_4005_s_65	11024181	( A) p53 recognises internal gaps in dsDNA oligonucleotides as short as 1 nt. Aliquots of 1 and 10 ng of unlabelled dsDNA oligonucleotides with internal single-strand gaps efficiently competed for p53 binding to the labelled ssDNA oligonucleotide NGC.	bind
58127	1	577	5	NULL	NULL	0	NULL	PABP	GP		does not bind			M161A		eIF4G	GP				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_1_104_s_93	15630022	( A) PABP M161A cannot bind to eIF4G.	bind
1766	1	577	6	NULL	NULL	0	NULL	PABP	GP		does not bind			M161A		eIF4G	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_1_104_s_93	15630022	( A) PABP M161A cannot bind to eIF4G.	bind
58128	1	579	5	NULL	NULL	0	NULL	PAX6	GP		does not bind					hGC 1BLs1 homologues	GP			B1 repetitive elements	NULL		NULL	NULL	NULL	NULL	gw60_gene_245_2_319_s_156	10717483	( A) PAX6 did not bind the hGC 1BLs1 homologues in the consensus B1 repetitive elements (lanes 3-5).	bind
1767	1	579	6	NULL	NULL	0	NULL	PAX6	GP		does not bind					hGC 1BLs1 homologue	GP			B1 repetitive element	NULL		NULL	NULL	NULL	NULL	gw60_gene_245_2_319_s_156	10717483	( A) PAX6 did not bind the hGC 1BLs1 homologues in the consensus B1 repetitive elements (lanes 3-5).	bind
58129	1	581	5	NULL	NULL	0	NULL	PCNA	GP		bind					GST-Cdt1	GP				NULL		0	NULL	NULL	NULL	gw70_embo_25_5_1126_s_196	16482215	( A) PCNA binds to GST-Cdt1, but not to GST.	bind
58130	2	581	5	NULL	NULL	0	NULL	PCNA	GP		does not bind					GST	Chemical				NULL		0	NULL	NULL	NULL	gw70_embo_25_5_1126_s_196	16482215	( A) PCNA binds to GST-Cdt1, but not to GST.	bind
1768	1	581	6	NULL	NULL	0	NULL	PCNA	GP		bind					GST-Cdt1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_5_1126_s_196	16482215	( A) PCNA binds to GST-Cdt1, but not to GST.	bind
58131	1	583	5	NULL	NULL	0	NULL	Socs-1	GP	phosphorylated	does not bind					Elongin BC	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_99_4_2175_s_184	11854514	( A) Phosphorylated Socs-1 does not bind Elongin BC as well as unphosphorylated Socs-1 in coimmunoprecipitation experiments.	bind
58132	2	583	5	NULL	NULL	0	NULL	Socs-1	GP	phosphorylated	does not bind					Socs-1	GP	unphosphorylated			NULL		0	NULL	NULL	NULL	gw60_pnas_99_4_2175_s_184	11854514	( A) Phosphorylated Socs-1 does not bind Elongin BC as well as unphosphorylated Socs-1 in coimmunoprecipitation experiments.	bind
1770	1	583	6	NULL	NULL	0	NULL	Socs-1	GP	phosphorylated	does not bind					Elongin BC	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_4_2175_s_184	11854514	( A) Phosphorylated Socs-1 does not bind Elongin BC as well as unphosphorylated Socs-1 in coimmunoprecipitation experiments.	bind
1772	2	583	6	NULL	NULL	0	NULL	Socs-1	GP	phosphorylated	does not bind					Socs-1	GP	unphosphorylated			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_4_2175_s_184	11854514	( A) Phosphorylated Socs-1 does not bind Elongin BC as well as unphosphorylated Socs-1 in coimmunoprecipitation experiments.	bind
58133	1	584	5	NULL	NULL	0	NULL	Pho4	GP		bind					Pse1	GP				NULL	extract	0	NULL	NULL	NULL	gw60_genesdev_12_17_2673_s_174	9732266	( A) Phosphorylation affects binding of Pho4 to Pse1 in an extract.	bind
58134	2	584	5	NULL	NULL	0	NULL	phosphorylation	Process		affects					statement 1	Process				NULL	extract	0	NULL	NULL	NULL	gw60_genesdev_12_17_2673_s_174	9732266	( A) Phosphorylation affects binding of Pho4 to Pse1 in an extract.	bind
1773	1	584	6	NULL	NULL	0	NULL	Pho4	GP		bind					Pse1	GP				NULL	extract	NULL	NULL	NULL	NULL	gw60_genesdev_12_17_2673_s_174	9732266	( A) Phosphorylation affects binding of Pho4 to Pse1 in an extract.	bind
1774	2	584	6	NULL	NULL	0	NULL	phosphorylation			affects					Statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_17_2673_s_174	9732266	( A) Phosphorylation affects binding of Pho4 to Pse1 in an extract.	bind
58135	1	585	5	NULL	NULL	0	NULL	PACS-1	GP		bind			MR		PACS-1	GP		FBR		NULL		0	NULL	NULL	NULL	gw70_embo_22_23_6234_s_87	14633983	( A) Phosphorylation of PACS-1 Ser278 inhibits PACS-1 MR binding to the PACS-1 FBR.	bind
58136	2	585	5	NULL	NULL	0	NULL	PACS-1	GP	phosphorylation of	inhibits			Ser278		statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_embo_22_23_6234_s_87	14633983	( A) Phosphorylation of PACS-1 Ser278 inhibits PACS-1 MR binding to the PACS-1 FBR.	bind
1775	1	585	6	NULL	NULL	0	NULL	PACS-1	GP		bind			MR		PACS-1	GP		FBR		NULL		NULL	NULL	NULL	NULL	gw70_embo_22_23_6234_s_87	14633983	( A) Phosphorylation of PACS-1 Ser278 inhibits PACS-1 MR binding to the PACS-1 FBR.	bind
1776	2	585	6	NULL	NULL	0	NULL	PACS-1	GP	phosphorylation	inhibit			Ser278		Statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_22_23_6234_s_87	14633983	( A) Phosphorylation of PACS-1 Ser278 inhibits PACS-1 MR binding to the PACS-1 FBR.	bind
58137	1	586	5	NULL	NULL	0	NULL	SRE	GP		mediates					gene expression	Process				NULL		0	NULL	NULL	NULL	gw60_embo_19_18_4955_s_67	10990459	( A) PI3K inhibitors decreased NGF-stimulated SRE-mediated gene expression.	bind
58138	2	586	5	NULL	NULL	0	NULL	NGF	GP		stimulates					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_embo_19_18_4955_s_67	10990459	( A) PI3K inhibitors decreased NGF-stimulated SRE-mediated gene expression.	bind
58139	3	586	5	NULL	NULL	0	NULL	PI3K inhibitors	GP		decreases					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_embo_19_18_4955_s_67	10990459	( A) PI3K inhibitors decreased NGF-stimulated SRE-mediated gene expression.	bind
58140	1	587	5	NULL	NULL	0	NULL	PIMT	GP		bind					AdoMet	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_98_18_10380_s_156	11517327	( A) PIMT binds AdoMet.	bind
1777	1	587	6	NULL	NULL	0	NULL	PIMT	GP		bind					AdoMet	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_18_10380_s_156	11517327	( A) PIMT binds AdoMet.	bind
58141	1	588	5	NULL	NULL	0	NULL	PIPK Igamma	GP		bind			mu2-subunit		AP-2	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_103_32_11934_s_90	16880396	( A) PIPK Igamma binds to AP-2 via its mu2-subunit.	bind
1778	1	588	6	NULL	NULL	0	NULL	PIPK Igamma	GP		bind			mu2-subunit		AP-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_32_11934_s_90	16880396	( A) PIPK Igamma binds to AP-2 via its mu2-subunit.	bind
58142	1	589	5	NULL	NULL	0	NULL	PML-RAR	GP		bind					RARbeta2	GP			promoter	NULL		0	NULL	NULL	NULL	gw60_science_295_5557_1079_s_31	11834837	( A) PML-RAR binds to the RARbeta2 promoter.	bind
1779	1	589	6	NULL	NULL	0	NULL	PML-RAR	GP		bind					RARbeta2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_science_295_5557_1079_s_31	11834837	( A) PML-RAR binds to the RARbeta2 promoter.	bind
58143	1	590	5	NULL	NULL	0	NULL	POT1b	GP		bind		efficiently			ss telomeric DNA	NucleicAcid			GGTTAGGGTTAG	NULL		0	NULL	NULL	NULL	gw70_embo_25_21_5180_s_66	17053789	( A) POT1b efficiently binds to a 12 base ss telomeric DNA sequence GGTTAGGGTTAG.	bind
1780	1	590	6	NULL	NULL	0	NULL	POT1b	GP		bind		efficiently			ss telomeric DNA sequence	NucleicAcid			GGTTAGGGTTAG	NULL		NULL	NULL	NULL	NULL	gw70_embo_25_21_5180_s_66	17053789	( A) POT1b efficiently binds to a 12 base ss telomeric DNA sequence GGTTAGGGTTAG.	bind
58144	1	591	5	NULL	NULL	0	NULL	PP1C	GP		bind					PTG	GP				NULL	in vivo	0	NULL	NULL	NULL	gw60_science_275_5305_1475_s_49	9045612	( A) PP1C binds PTG in vivo.	bind
1781	1	591	6	NULL	NULL	0	NULL	PP1C	GP		bind					PTG	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_science_275_5305_1475_s_49	9045612	( A) PP1C binds PTG in vivo.	bind
58145	1	592	5	NULL	NULL	0	NULL				bind				PRE				PHO		NULL		0	NULL	NULL	NULL	gw70_genesdev_19_15_1755_s_68	16077005	( A) PRE binding of PHO, deltaPBD and PCC was studied by bandshift assays.	bind
58146	2	592	5	NULL	NULL	0	NULL				bind				PRE				deltaPBD		NULL		0	NULL	NULL	NULL	gw70_genesdev_19_15_1755_s_68	16077005	( A) PRE binding of PHO, deltaPBD and PCC was studied by bandshift assays.	bind
58147	3	592	5	NULL	NULL	0	NULL				bind				PRE				PCC		NULL		0	NULL	NULL	NULL	gw70_genesdev_19_15_1755_s_68	16077005	( A) PRE binding of PHO, deltaPBD and PCC was studied by bandshift assays.	bind
1782	1	592	6	NULL	NULL	0	NULL		AminoAcid		bind			PHO			GP			PRE	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_15_1755_s_68	16077005	( A) PRE binding of PHO, deltaPBD and PCC was studied by bandshift assays.	bind
1783	2	592	6	NULL	NULL	0	NULL		AminoAcid		bind			deltaPBD			GP			PRE	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_15_1755_s_68	16077005	( A) PRE binding of PHO, deltaPBD and PCC was studied by bandshift assays.	bind
1784	3	592	6	NULL	NULL	0	NULL		AminoAcid		bind			PCC			GP			PRE	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_15_1755_s_68	16077005	( A) PRE binding of PHO, deltaPBD and PCC was studied by bandshift assays.	bind
58148	1	593	5	NULL	NULL	0	NULL	FN	GP		is					fibronectin	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_46_16210_s_148	15520390	( A) Primary rat and human VSMC adhered to Netrin-1 and fibronectin (FN), whereas HAEC  and HMVEC did not adhere to the Netrin-1, but bound tightly to FN.	bind
58149	2	593	5	NULL	NULL	0	NULL	primary VSMC	Cell	rat	adhere to					Netrin-1	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_46_16210_s_148	15520390	( A) Primary rat and human VSMC adhered to Netrin-1 and fibronectin (FN), whereas HAEC  and HMVEC did not adhere to the Netrin-1, but bound tightly to FN.	bind
58150	3	593	5	NULL	NULL	0	NULL	primary VSMC	Cell	human	adhere to					Netrin-1	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_46_16210_s_148	15520390	( A) Primary rat and human VSMC adhered to Netrin-1 and fibronectin (FN), whereas HAEC  and HMVEC did not adhere to the Netrin-1, but bound tightly to FN.	bind
58151	4	593	5	NULL	NULL	0	NULL	primary VSMC	Cell	rat	adhere to					FN	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_46_16210_s_148	15520390	( A) Primary rat and human VSMC adhered to Netrin-1 and fibronectin (FN), whereas HAEC  and HMVEC did not adhere to the Netrin-1, but bound tightly to FN.	bind
58152	5	593	5	NULL	NULL	0	NULL	primary VSMC	Cell	human	adhere to					FN	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_46_16210_s_148	15520390	( A) Primary rat and human VSMC adhered to Netrin-1 and fibronectin (FN), whereas HAEC  and HMVEC did not adhere to the Netrin-1, but bound tightly to FN.	bind
58153	6	593	5	NULL	NULL	0	NULL	HAEC	Cell		does not adhere to					Netrin-1	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_46_16210_s_148	15520390	( A) Primary rat and human VSMC adhered to Netrin-1 and fibronectin (FN), whereas HAEC  and HMVEC did not adhere to the Netrin-1, but bound tightly to FN.	bind
58154	7	593	5	NULL	NULL	0	NULL	HMVEC	Cell		does not adhere to					Netrin-1	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_46_16210_s_148	15520390	( A) Primary rat and human VSMC adhered to Netrin-1 and fibronectin (FN), whereas HAEC  and HMVEC did not adhere to the Netrin-1, but bound tightly to FN.	bind
58155	8	593	5	NULL	NULL	0	NULL	HAEC	Cell		bind		tightly			FN	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_46_16210_s_148	15520390	( A) Primary rat and human VSMC adhered to Netrin-1 and fibronectin (FN), whereas HAEC  and HMVEC did not adhere to the Netrin-1, but bound tightly to FN.	bind
58156	9	593	5	NULL	NULL	0	NULL	HMVEC	Cell		bind		tightly			FN	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_46_16210_s_148	15520390	( A) Primary rat and human VSMC adhered to Netrin-1 and fibronectin (FN), whereas HAEC  and HMVEC did not adhere to the Netrin-1, but bound tightly to FN.	bind
1785	1	593	6	NULL	NULL	0	NULL	primary VSMC	Cell	rat	adhere					Netrin-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_46_16210_s_148	15520390	( A) Primary rat and human VSMC adhered to Netrin-1 and fibronectin (FN), whereas HAEC  and HMVEC did not adhere to the Netrin-1, but bound tightly to FN.	bind
1786	2	593	6	NULL	NULL	0	NULL	primary VSMC	Cell	human	adhere					fibronectin 	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_46_16210_s_148	15520390	( A) Primary rat and human VSMC adhered to Netrin-1 and fibronectin (FN), whereas HAEC  and HMVEC did not adhere to the Netrin-1, but bound tightly to FN.	bind
1787	3	593	6	NULL	NULL	0	NULL	primary VSMC	Cell	rat	adhere					fibronectin 	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_46_16210_s_148	15520390	( A) Primary rat and human VSMC adhered to Netrin-1 and fibronectin (FN), whereas HAEC  and HMVEC did not adhere to the Netrin-1, but bound tightly to FN.	bind
1788	4	593	6	NULL	NULL	0	NULL	primary VSMC	Cell	human	adhere					Netrin-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_46_16210_s_148	15520390	( A) Primary rat and human VSMC adhered to Netrin-1 and fibronectin (FN), whereas HAEC  and HMVEC did not adhere to the Netrin-1, but bound tightly to FN.	bind
1789	5	593	6	NULL	NULL	0	NULL	HAEC	Cell		did not adhere					Netrin1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_46_16210_s_148	15520390	( A) Primary rat and human VSMC adhered to Netrin-1 and fibronectin (FN), whereas HAEC  and HMVEC did not adhere to the Netrin-1, but bound tightly to FN.	bind
1790	6	593	6	NULL	NULL	0	NULL	HMVEC	Cell		did not adhere					Netrin-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_46_16210_s_148	15520390	( A) Primary rat and human VSMC adhered to Netrin-1 and fibronectin (FN), whereas HAEC  and HMVEC did not adhere to the Netrin-1, but bound tightly to FN.	bind
1791	7	593	6	NULL	NULL	0	NULL	HAEC	Cell		bind		tightly			FN	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_46_16210_s_148	15520390	( A) Primary rat and human VSMC adhered to Netrin-1 and fibronectin (FN), whereas HAEC  and HMVEC did not adhere to the Netrin-1, but bound tightly to FN.	bind
1792	8	593	6	NULL	NULL	0	NULL	HMVEC	Cell		bind		tightly			FN	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_46_16210_s_148	15520390	( A) Primary rat and human VSMC adhered to Netrin-1 and fibronectin (FN), whereas HAEC  and HMVEC did not adhere to the Netrin-1, but bound tightly to FN.	bind
58157	1	594	5	NULL	NULL	0	NULL	Prolyl-sulfamoyl-adenylate	Chemical		bind					ProRS	GP	M. thermautotrophicus	active site		NULL		0	NULL	NULL	NULL	gw60_pnas_100_4_1673_s_125	12578991	( a) Prolyl-sulfamoyl-adenylate bound to the active site of  M. thermautotrophicus ProRS.	bind
1793	1	594	6	NULL	NULL	0	NULL		AminoAcid		bind			Prolyl-sulfamoyl-adenylate		ProRS	GP	M. thermautotrophicus	active site		NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_4_1673_s_125	12578991	( a) Prolyl-sulfamoyl-adenylate bound to the active site of  M. thermautotrophicus ProRS.	bind
58158	1	595	5	NULL	NULL	0	NULL	Protein G	GP		bind					IgG Fc fragment	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_99_22_14116_s_118	12381794	( a) Protein G bound to an IgG Fc fragment (1fcc).	bind
58159	2	595	5	NULL	NULL	0	NULL	IgG Fc fragment	GP		is					1fcc	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_99_22_14116_s_118	12381794	( a) Protein G bound to an IgG Fc fragment (1fcc).	bind
1794	1	595	6	NULL	NULL	0	NULL	Protein G	GP		bind					IgG 	GP		Fc fragment		NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_22_14116_s_118	12381794	( a) Protein G bound to an IgG Fc fragment (1fcc).	bind
58160	1	596	5	NULL	NULL	0	NULL	Protein sigma1	GP		bind					NALT M cells	Cell				NULL		0	NULL	NULL	NULL	gw60_pnas_98_16_9318_s_94	11459939	( A) Protein sigma1 (yellow arrows) and UEA-1 (white arrows) binding to NALT M cells at x180.	bind
58161	2	596	5	NULL	NULL	0	NULL	UEA-1	GP		bind					NALT M cells	Cell				NULL		0	NULL	NULL	NULL	gw60_pnas_98_16_9318_s_94	11459939	( A) Protein sigma1 (yellow arrows) and UEA-1 (white arrows) binding to NALT M cells at x180.	bind
1795	1	596	6	NULL	NULL	0	NULL	Protein sigma1	GP		bind					NALT M cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_16_9318_s_94	11459939	( A) Protein sigma1 (yellow arrows) and UEA-1 (white arrows) binding to NALT M cells at x180.	bind
1796	2	596	6	NULL	NULL	0	NULL	UEA-1	GP		bind					NALT M cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_16_9318_s_94	11459939	( A) Protein sigma1 (yellow arrows) and UEA-1 (white arrows) binding to NALT M cells at x180.	bind
58162	1	598	5	NULL	NULL	0	NULL	pTP	GP		bind								TD(30 - 50)		NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_12_3274_s_134	12799455	( A) pTP binding to TD(30 - 50) was studied using EMSA.	bind
1797	1	598	6	NULL	NULL	0	NULL	pTP	GP		bind						AminoAcid		TD (30-50)		NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_12_3274_s_134	12799455	( A) pTP binding to TD(30 - 50) was studied using EMSA.	bind
58163	1	601	5	NULL	NULL	0	NULL	myosin	GP	purified	bind					P210 BCR-ABL	GP	expressed in;;purified from Sf9 cells			NULL		0	NULL	NULL	NULL	gw60_pnas_96_1_203_s_103	9874796	( a) Purified myosin (0.2 mug) (lane 1) and GST-C32 bound to P210 BCR-ABL (lane 2) expressed in and purified from Sf9 cells were stained by silver nitrate.	bind
58164	2	601	5	NULL	NULL	0	NULL	GST-C32	GP		bind					P210 BCR-ABL	GP	expressed in;;purified from Sf9 cells			NULL		0	NULL	NULL	NULL	gw60_pnas_96_1_203_s_103	9874796	( a) Purified myosin (0.2 mug) (lane 1) and GST-C32 bound to P210 BCR-ABL (lane 2) expressed in and purified from Sf9 cells were stained by silver nitrate.	bind
1905	1	601	6	NULL	NULL	0	NULL	myosin	GP	purified	bind					P210 BCR-ABL	GP				NULL	Sf9 cells	NULL	NULL	NULL	NULL	gw60_pnas_96_1_203_s_103	9874796	( a) Purified myosin (0.2 mug) (lane 1) and GST-C32 bound to P210 BCR-ABL (lane 2) expressed in and purified from Sf9 cells were stained by silver nitrate.	bind
1906	2	601	6	NULL	NULL	0	NULL	GST-C32	GP		bind					P210 BCR-ABL	GP				NULL	Sf9 cells	NULL	NULL	NULL	NULL	gw60_pnas_96_1_203_s_103	9874796	( a) Purified myosin (0.2 mug) (lane 1) and GST-C32 bound to P210 BCR-ABL (lane 2) expressed in and purified from Sf9 cells were stained by silver nitrate.	bind
58165	1	602	5	NULL	NULL	0	NULL	Pyr	GP		bind					PvDHFR	GP	WT			NULL		0	NULL	NULL	NULL	gw70_pnas_102_37_13046_s_97	16135570	( A) Pyr binding with the WT PvDHFR.	bind
2082	1	602	6	NULL	NULL	0	NULL	Pyr	GP		bind					PvDHFR	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_37_13046_s_97	16135570	( A) Pyr binding with the WT PvDHFR.	bind
57	1	602	9	10	NULL	0	NULL	Pyr	NULL		bind	NULL				 PvDHFR	NULL	WT			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_37_13046_s_97	16135570	( A) Pyr binding with the WT PvDHFR.	bind
58166	1	603	5	NULL	NULL	0	NULL	FGF2	GP		bind					heparin	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_14_4833_s_168	15051888	( A) QSulf1 does not affect the binding of FGF2 to heparin.	bind
58167	2	603	5	NULL	NULL	0	NULL	QSulf1	GP		does not affect					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_101_14_4833_s_168	15051888	( A) QSulf1 does not affect the binding of FGF2 to heparin.	bind
2083	1	603	6	NULL	NULL	0	NULL	FGF2	GP		bind					heparin	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_14_4833_s_168	15051888	( A) QSulf1 does not affect the binding of FGF2 to heparin.	bind
2084	2	603	6	NULL	NULL	0	NULL	Qsulf1	GP		does not affect					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_14_4833_s_168	15051888	( A) QSulf1 does not affect the binding of FGF2 to heparin.	bind
58	1	603	9	NULL	NULL	0	NULL	FGF2	NULL		bind	NULL				heparin	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_101_14_4833_s_168	15051888	( A) QSulf1 does not affect the binding of FGF2 to heparin.	bind
59	2	603	9	NULL	NULL	0	NULL	QSulf1	NULL		does not affect	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_101_14_4833_s_168	15051888	( A) QSulf1 does not affect the binding of FGF2 to heparin.	bind
58168	1	605	5	NULL	NULL	0	NULL	Fz proteins	GP		activates					Rac	GP				NULL		0	NULL	NULL	NULL	gw60_genesdev_17_2_295_s_51	12533515	( A) Rac activation by specific Fz proteins.	bind
2085	1	605	6	NULL	NULL	0	NULL	Fz proteins	GP	specific	activates					Rac	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_2_295_s_51	12533515	( A) Rac activation by specific Fz proteins.	bind
60	1	605	9	10	NULL	0	NULL	Fz proteins	NULL		activates	NULL				Rac	NULL				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_2_295_s_51	12533515	( A) Rac activation by specific Fz proteins.	bind
61	1	606	9	NULL	NULL	0	NULL	SRP54	NULL	Radiolabeled 	bind	NULL				RNC-pPL86	NULL				NULL		0	NULL	NULL	NULL	gw60_science_297_5585_1345_s_55	12193787	( A) Radiolabeled SRP54 was bound to RNC-pPL86 and then treated with DSS.	bind
58169	1	608	5	NULL	NULL	0	NULL	RASSF1	GP		bind					Daxx	GP				NULL	COS7 cells	0	NULL	NULL	NULL	gw70_embo_25_14_3286_s_83	16810318	( A) RASSF1 binds Daxx in COS7 cells.	bind
1798	1	608	6	NULL	NULL	0	NULL	RASSF1	GP		bind					Daxx	GP				NULL	Cos7 cells	NULL	NULL	NULL	NULL	gw70_embo_25_14_3286_s_83	16810318	( A) RASSF1 binds Daxx in COS7 cells.	bind
58170	1	609	5	NULL	NULL	0	NULL	GABAAR beta3	GP	rat	bind					BTX	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_52	16549768	( a) Rat (r) GABAAR beta3 binds BTX, but rat GABAAR beta1, beta2, alpha2, and gamma2 do not.	bind
58171	2	609	5	NULL	NULL	0	NULL	GABAAR beta1	GP	rat	does not bind					BTX	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_52	16549768	( a) Rat (r) GABAAR beta3 binds BTX, but rat GABAAR beta1, beta2, alpha2, and gamma2 do not.	bind
58172	3	609	5	NULL	NULL	0	NULL	GABAAR beta2	GP	rat	does not bind					BTX	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_52	16549768	( a) Rat (r) GABAAR beta3 binds BTX, but rat GABAAR beta1, beta2, alpha2, and gamma2 do not.	bind
58173	4	609	5	NULL	NULL	0	NULL	GABAAR alpha2	GP	rat	does not bind					BTX	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_52	16549768	( a) Rat (r) GABAAR beta3 binds BTX, but rat GABAAR beta1, beta2, alpha2, and gamma2 do not.	bind
58174	5	609	5	NULL	NULL	0	NULL	GABAAR gamma2	GP	rat	does not bind					BTX	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_52	16549768	( a) Rat (r) GABAAR beta3 binds BTX, but rat GABAAR beta1, beta2, alpha2, and gamma2 do not.	bind
1799	1	609	6	NULL	NULL	0	NULL	GABAAR beta3	GP	rat	bind					BTX	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_52	16549768	( a) Rat (r) GABAAR beta3 binds BTX, but rat GABAAR beta1, beta2, alpha2, and gamma2 do not.	bind
1800	2	609	6	NULL	NULL	0	NULL	GABAAR beta1	GP	rat	does not bind					BTX	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_52	16549768	( a) Rat (r) GABAAR beta3 binds BTX, but rat GABAAR beta1, beta2, alpha2, and gamma2 do not.	bind
1801	3	609	6	NULL	NULL	0	NULL	GABAAR beta2	GP	rat	does not bind					BTX	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_52	16549768	( a) Rat (r) GABAAR beta3 binds BTX, but rat GABAAR beta1, beta2, alpha2, and gamma2 do not.	bind
1802	4	609	6	NULL	NULL	0	NULL	GABAAR alpha2	GP	rat	does not bind					BTX	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_52	16549768	( a) Rat (r) GABAAR beta3 binds BTX, but rat GABAAR beta1, beta2, alpha2, and gamma2 do not.	bind
1803	5	609	6	NULL	NULL	0	NULL	GABAAR gamma2	GP	rat	does not bind					BTX	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_52	16549768	( a) Rat (r) GABAAR beta3 binds BTX, but rat GABAAR beta1, beta2, alpha2, and gamma2 do not.	bind
58175	1	611	5	NULL	NULL	0	NULL	Rbx1	GP		bind					Cdc34	GP				NULL	insect cells	0	NULL	NULL	NULL	gw60_science_284_5414_662_s_87	10213692	( A) Rbx1 binds Cdc34 and stimulates association of Cdc53 with Cdc34 in insect cells.	bind
58176	2	611	5	NULL	NULL	0	NULL	Cdc53	GP		associate with					Cdc34	GP				NULL	insect cells	0	NULL	NULL	NULL	gw60_science_284_5414_662_s_87	10213692	( A) Rbx1 binds Cdc34 and stimulates association of Cdc53 with Cdc34 in insect cells.	bind
58177	3	611	5	NULL	NULL	0	NULL	statement 1	Process		stimulates					statement 2	Process				NULL	insect cells	0	NULL	NULL	NULL	gw60_science_284_5414_662_s_87	10213692	( A) Rbx1 binds Cdc34 and stimulates association of Cdc53 with Cdc34 in insect cells.	bind
1827	1	611	6	NULL	NULL	0	NULL	Rbx1	GP		bind					Cdc34	GP				NULL	insect cells	NULL	NULL	NULL	NULL	gw60_science_284_5414_662_s_87	10213692	( A) Rbx1 binds Cdc34 and stimulates association of Cdc53 with Cdc34 in insect cells.	bind
1828	2	611	6	NULL	NULL	0	NULL	Cdc53	GP		bind					Cdc34	GP				NULL	insect cells	NULL	NULL	NULL	NULL	gw60_science_284_5414_662_s_87	10213692	( A) Rbx1 binds Cdc34 and stimulates association of Cdc53 with Cdc34 in insect cells.	bind
1829	3	611	6	NULL	NULL	0	NULL	Statement 1	Process		stimulate					Statement 2	Process				NULL	insect cells	NULL	NULL	NULL	NULL	gw60_science_284_5414_662_s_87	10213692	( A) Rbx1 binds Cdc34 and stimulates association of Cdc53 with Cdc34 in insect cells.	bind
58178	1	612	5	NULL	NULL	0	NULL	Sp-1	GP	endogenous	bind					M-CSF	GP			promoter	NULL		0	NULL	NULL	NULL	gw60_jclininvest_102_10_1850_s_203	9819371	( A) Recombinant Egr-1 decreases the binding of endogenous Sp-1 and Sp-3 from the M-CSF promoter.	bind
58179	2	612	5	NULL	NULL	0	NULL	Sp-3	GP	endogenous	bind					M-CSF	GP			promoter	NULL		0	NULL	NULL	NULL	gw60_jclininvest_102_10_1850_s_203	9819371	( A) Recombinant Egr-1 decreases the binding of endogenous Sp-1 and Sp-3 from the M-CSF promoter.	bind
58180	3	612	5	NULL	NULL	0	NULL	Egr-1	GP	recombinant	decreases					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jclininvest_102_10_1850_s_203	9819371	( A) Recombinant Egr-1 decreases the binding of endogenous Sp-1 and Sp-3 from the M-CSF promoter.	bind
58181	4	612	5	NULL	NULL	0	NULL	Egr-1	GP	recombinant	decreases					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jclininvest_102_10_1850_s_203	9819371	( A) Recombinant Egr-1 decreases the binding of endogenous Sp-1 and Sp-3 from the M-CSF promoter.	bind
1830	1	612	6	NULL	NULL	0	NULL	Sp1	GP	endogenous	bind					M-CSF 	GP			Promoter	NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_10_1850_s_203	9819371	( A) Recombinant Egr-1 decreases the binding of endogenous Sp-1 and Sp-3 from the M-CSF promoter.	bind
1831	2	612	6	NULL	NULL	0	NULL	Sp3	GP	endogenous	bind					M-CSF 	GP			Promoter	NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_10_1850_s_203	9819371	( A) Recombinant Egr-1 decreases the binding of endogenous Sp-1 and Sp-3 from the M-CSF promoter.	bind
1832	3	612	6	NULL	NULL	0	NULL	Egr-1	GP	recombinant	decreases					Statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_10_1850_s_203	9819371	( A) Recombinant Egr-1 decreases the binding of endogenous Sp-1 and Sp-3 from the M-CSF promoter.	bind
1833	4	612	6	NULL	NULL	0	NULL	Egr-1	GP	recombinant	decreases					Statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_10_1850_s_203	9819371	( A) Recombinant Egr-1 decreases the binding of endogenous Sp-1 and Sp-3 from the M-CSF promoter.	bind
58182	1	616	5	NULL	NULL	0	NULL	RelA	GP		bind					p300	GP		amino acid residues (1-610)		NULL		0	NULL	NULL	NULL	gw60_embo_17_11_3124_s_36	9606194	( A) RelA binds p300 between amino acid residues 1 and 610.	bind
1834	1	616	6	NULL	NULL	0	NULL	RelA	GP		bind					p300	GP		 amino acid residues 1 and 610		NULL		NULL	NULL	NULL	NULL	gw60_embo_17_11_3124_s_36	9606194	( A) RelA binds p300 between amino acid residues 1 and 610.	bind
58183	1	620	5	NULL	NULL	0	NULL	RFC	GP		forms complex with					Asf1	GP				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1365_s_210	15901673	( A) RFC and Rfc2-5 coprecipitate with Asf1.	bind
58184	2	620	5	NULL	NULL	0	NULL	Rfc2	GP		forms complex with					Asf1	GP				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1365_s_210	15901673	( A) RFC and Rfc2-5 coprecipitate with Asf1.	bind
58185	3	620	5	NULL	NULL	0	NULL	Rfc3	GP		forms complex with					Asf1	GP				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1365_s_210	15901673	( A) RFC and Rfc2-5 coprecipitate with Asf1.	bind
58186	4	620	5	NULL	NULL	0	NULL	Rfc4	GP		forms complex with					Asf1	GP				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1365_s_210	15901673	( A) RFC and Rfc2-5 coprecipitate with Asf1.	bind
58187	5	620	5	NULL	NULL	0	NULL	Rfc5	GP		forms complex with					Asf1	GP				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1365_s_210	15901673	( A) RFC and Rfc2-5 coprecipitate with Asf1.	bind
1835	1	620	6	NULL	NULL	0	NULL	RFC	GP		bind					Asf1	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_11_1365_s_210	15901673	( A) RFC and Rfc2-5 coprecipitate with Asf1.	bind
1836	2	620	6	NULL	NULL	0	NULL	Rfc2-5	GP		bind					Asf1	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_11_1365_s_210	15901673	( A) RFC and Rfc2-5 coprecipitate with Asf1.	bind
58188	1	622	5	NULL	NULL	0	NULL	RAR	GP		bind					all- trans retinoic acid	Chemical				NULL		0	NULL	NULL	NULL	gw60_annrevbiochem_68_0_559_s_136	10872460	( a) Ribbon diagram of RAR bound to   all- trans retinoic acid ( red).	bind
1837	1	622	6	NULL	NULL	0	NULL	RAR	GP		bind					 all- trans retinoic acid	GP				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_68_0_559_s_136	10872460	( a) Ribbon diagram of RAR bound to   all- trans retinoic acid ( red).	bind
58189	1	623	5	NULL	NULL	0	NULL	14-3-3c protein dimer	GP	 tobacco	bind					peptide Gln-Ser-Tyr-pThr-Val	AminoAcid				NULL		0	NULL	NULL	NULL	gw70_embo_22_5_987_s_34	12606564	( A) Ribbon plot of two different orientations of the dimeric tobacco 14-3-3c protein  (green) bound to the peptide Gln-Ser-Tyr-pThr-Val (yellow), which constitutes the  C-terminal end of PMA2, a H+-ATPase isoform from  Nicotiana plumbaginifolia.	bind
58190	2	623	5	NULL	NULL	0	NULL	peptide Gln-Ser-Tyr-pThr-Val	AminoAcid		constitutes					PMA2	GP		C-terminal end		NULL		0	NULL	NULL	NULL	gw70_embo_22_5_987_s_34	12606564	( A) Ribbon plot of two different orientations of the dimeric tobacco 14-3-3c protein  (green) bound to the peptide Gln-Ser-Tyr-pThr-Val (yellow), which constitutes the  C-terminal end of PMA2, a H+-ATPase isoform from  Nicotiana plumbaginifolia.	bind
58191	3	623	5	NULL	NULL	0	NULL	PMA2	GP		is an isoform of					H+-ATPase	GP	Nicotiana plumbaginifolia			NULL		0	NULL	NULL	NULL	gw70_embo_22_5_987_s_34	12606564	( A) Ribbon plot of two different orientations of the dimeric tobacco 14-3-3c protein  (green) bound to the peptide Gln-Ser-Tyr-pThr-Val (yellow), which constitutes the  C-terminal end of PMA2, a H+-ATPase isoform from  Nicotiana plumbaginifolia.	bind
58192	1	625	5	NULL	NULL	0	NULL	3G ARNO	GP		bind			PH domain		Ins(1,4,5)P3	Chemical				NULL		0	NULL	NULL	NULL	gw70_embo_23_19_3711_s_40	15359279	( A) Ribbon representation of the 3G ARNO PH domain bound to Ins(1,4,5)P3.	bind
1838	1	625	6	3	NULL	0	NULL	3G ARNO	GP		bind			 PH domain		Ins(1,4,5)P3	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_19_3711_s_40	15359279	( A) Ribbon representation of the 3G ARNO PH domain bound to Ins(1,4,5)P3.	bind
58193	1	626	5	NULL	NULL	0	NULL	RLF	GP		is activated during					metaphase-anaphase transition	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_139_1_13_s_155	9314525	( a) RLF becomes active at  metaphase-anaphase transition;  Drosophila MCMs binding to chromosomes follows metaphase-anaphase transition.	bind
58194	2	626	5	NULL	NULL	0	NULL	MCMs	GP	Drosophila	bind					chromosomes	Chromosome				NULL		0	NULL	NULL	NULL	gw60_cellbiol_139_1_13_s_155	9314525	( a) RLF becomes active at  metaphase-anaphase transition;  Drosophila MCMs binding to chromosomes follows metaphase-anaphase transition.	bind
58195	3	626	5	NULL	NULL	0	NULL	statement 2	Process		follows					metaphase-anaphase transition	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_139_1_13_s_155	9314525	( a) RLF becomes active at  metaphase-anaphase transition;  Drosophila MCMs binding to chromosomes follows metaphase-anaphase transition.	bind
1839	1	626	6	NULL	NULL	0	NULL	MCMs	GP	Drosophila	bind					chromosomes	Chromosome				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_139_1_13_s_155	9314525	( a) RLF becomes active at  metaphase-anaphase transition;  Drosophila MCMs binding to chromosomes follows metaphase-anaphase transition.	bind
1840	2	626	6	NULL	NULL	0	NULL	Statement 1	Process		follows					metaphase-anaphase 	Process	transition of			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_139_1_13_s_155	9314525	( a) RLF becomes active at  metaphase-anaphase transition;  Drosophila MCMs binding to chromosomes follows metaphase-anaphase transition.	bind
1841	3	626	6	NULL	NULL	0	NULL	RLF	GP		is active at					metaphase-anaphase 	Process	transition of			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_139_1_13_s_155	9314525	( a) RLF becomes active at  metaphase-anaphase transition;  Drosophila MCMs binding to chromosomes follows metaphase-anaphase transition.	bind
58196	1	628	5	NULL	NULL	0	NULL	Salp	GP		bind					p85	GP		SH3 domain		NULL		0	NULL	NULL	NULL	gw60_gene_240_1_133_s_248	10564820	( A) Salp  binds the p85 SH3 domain.	bind
1842	1	628	6	NULL	NULL	0	NULL	Salp	GP		bind					p85	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_gene_240_1_133_s_248	10564820	( A) Salp  binds the p85 SH3 domain.	bind
58197	1	630	5	NULL	NULL	0	NULL	PDK1	GP		bind					PtdIns(3,4,5)P3	Chemical	biotinylated			NULL		0	NULL	NULL	NULL	gw70_embo_23_20_3918_s_171	15457207	( A) Saturation-binding isotherms of the indicated forms of PDK1 binding to biotinylated-PtdIns(3,4,5)P3 (bPIP3).	bind
58198	2	630	5	NULL	NULL	0	NULL	biotinylated-PtdIns(3,4,5)P3	Chemical		is					bPIP3	Chemical				NULL		0	NULL	NULL	NULL	gw70_embo_23_20_3918_s_171	15457207	( A) Saturation-binding isotherms of the indicated forms of PDK1 binding to biotinylated-PtdIns(3,4,5)P3 (bPIP3).	bind
1865	1	630	6	NULL	NULL	0	NULL	PDK1	GP		bind					PtdIns(3,4,5)P3 (bPIP3)	GP	biotinylated			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_20_3918_s_171	15457207	( A) Saturation-binding isotherms of the indicated forms of PDK1 binding to biotinylated-PtdIns(3,4,5)P3 (bPIP3).	bind
58199	1	631	5	NULL	NULL	0	NULL	NT-3	GP	iodinated	bind					Ltrk	Cell				NULL		0	NULL	NULL	NULL	gw60_embo_17_9_2534_s_134	9564036	( A) Scatchard analyses of saturation curves for iodinated NT-3 binding to the Ltrk fibroblast cell line.	bind
58200	2	631	5	NULL	NULL	0	NULL	Ltrk	Cell		is a type of					fibroblast cell line	Cell				NULL		0	NULL	NULL	NULL	gw60_embo_17_9_2534_s_134	9564036	( A) Scatchard analyses of saturation curves for iodinated NT-3 binding to the Ltrk fibroblast cell line.	bind
1871	1	631	6	NULL	NULL	0	NULL	NT-3	GP	iodinated	bind					Ltrk	Cell				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_9_2534_s_134	9564036	( A) Scatchard analyses of saturation curves for iodinated NT-3 binding to the Ltrk fibroblast cell line.	bind
51837	2	631	6	NULL	NULL	0	NULL	 Ltrk	Cell		is a type of					fibroblast cell line	Cell				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_9_2534_s_134	9564036	( A) Scatchard analyses of saturation curves for iodinated NT-3 binding to the Ltrk fibroblast cell line.	bind
58201	1	632	5	NULL	NULL	0	NULL	EGF	GP		bind					MDCK-EGFR cells	Cell				NULL		0	NULL	NULL	NULL	gw70_embo_23_8_1739_s_83	15057284	( A) Scatchard analysis of EGF binding to MDCK-EGFR cells.	bind
1872	1	632	6	NULL	NULL	0	NULL	EGF 	GP		bind					MDCK-EGFR cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_8_1739_s_83	15057284	( A) Scatchard analysis of EGF binding to MDCK-EGFR cells.	bind
58202	1	641	5	NULL	NULL	0	NULL	MBP-CTD	GP		bind					TBP	GP				NULL	in vitro	0	NULL	NULL	NULL	gw70_pnas_100_17_10108_s_181	12900506	( A) SDS/PAGE analysis of  in vitro protein interactions shows  that MBP-CTD binds TBP, but not VirD2, whereas VirD2  recruits TBP.	bind
58203	2	641	5	NULL	NULL	0	NULL	MBP-CTD	GP		does not bind					VirD2	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_100_17_10108_s_181	12900506	( A) SDS/PAGE analysis of  in vitro protein interactions shows  that MBP-CTD binds TBP, but not VirD2, whereas VirD2  recruits TBP.	bind
58204	3	641	5	NULL	NULL	0	NULL	VirD2	GP		recruit					TBP	GP				NULL	in vitro	0	NULL	NULL	NULL	gw70_pnas_100_17_10108_s_181	12900506	( A) SDS/PAGE analysis of  in vitro protein interactions shows  that MBP-CTD binds TBP, but not VirD2, whereas VirD2  recruits TBP.	bind
1873	1	641	6	NULL	NULL	0	NULL	MBP	GP		bind			CTD		TBP	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_100_17_10108_s_181	12900506	( A) SDS/PAGE analysis of  in vitro protein interactions shows  that MBP-CTD binds TBP, but not VirD2, whereas VirD2  recruits TBP.	bind
1874	2	641	6	NULL	NULL	0	NULL	MBP	GP		does not bind			CTD		VirD2	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_100_17_10108_s_181	12900506	( A) SDS/PAGE analysis of  in vitro protein interactions shows  that MBP-CTD binds TBP, but not VirD2, whereas VirD2  recruits TBP.	bind
1875	3	641	6	NULL	NULL	0	NULL	VirD2	GP		recruits					TBP	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_100_17_10108_s_181	12900506	( A) SDS/PAGE analysis of  in vitro protein interactions shows  that MBP-CTD binds TBP, but not VirD2, whereas VirD2  recruits TBP.	bind
58205	1	642	5	NULL	NULL	0	NULL	WCE	GP	yeast	bind					ScOrc4p	GP	His6-tagged			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_9_4938_s_178	11296251	( a) SDS/PAGE of proteins from yeast WCE bound to Ni2+-Sepharose saturated with His6-tagged ScOrc4p or RepA (major bands).	bind
58206	2	642	5	NULL	NULL	0	NULL	WCE	GP	yeast	bind					RepA	GP	His6-tagged			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_9_4938_s_178	11296251	( a) SDS/PAGE of proteins from yeast WCE bound to Ni2+-Sepharose saturated with His6-tagged ScOrc4p or RepA (major bands).	bind
58207	3	642	5	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_9_4938_s_178	11296251	( a) SDS/PAGE of proteins from yeast WCE bound to Ni2+-Sepharose saturated with His6-tagged ScOrc4p or RepA (major bands).	bind
1876	1	642	6	NULL	NULL	0	NULL	WCE	GP	yeast	bind					ScOrc4p 	GP	His6-tagged			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_9_4938_s_178	11296251	( a) SDS/PAGE of proteins from yeast WCE bound to Ni2+-Sepharose saturated with His6-tagged ScOrc4p or RepA (major bands).	bind
58208	1	643	5	NULL	NULL	0	NULL	Sec23-24p	GP		bind					Bet1p	GP		COOH-terminal (membrane-proximal) 79 amino acids of the cytosolic domain		NULL		0	NULL	NULL	NULL	gw60_science_281_5377_698_s_77	9685263	( A) Sec23-24p binding is localized to the COOH-terminal (membrane-proximal) 79 amino acids of the cytosolic domain of Bet1p, whereas Sar1p can bind to the 41 COOH-terminal amino acids of the cytosolic domain.	bind
58209	2	643	5	NULL	NULL	0	NULL	Sar1p	GP		bind					Bet1p	GP		COOH-terminal amino acids of cytosolic domain		NULL		0	NULL	NULL	NULL	gw60_science_281_5377_698_s_77	9685263	( A) Sec23-24p binding is localized to the COOH-terminal (membrane-proximal) 79 amino acids of the cytosolic domain of Bet1p, whereas Sar1p can bind to the 41 COOH-terminal amino acids of the cytosolic domain.	bind
1877	1	643	6	NULL	NULL	0	NULL	Sec23-24p	GP		bind					Bet1p	GP		COOH-terminal (membrane-proximal) 79 amino acids of the cytosolic domain		NULL		NULL	NULL	NULL	NULL	gw60_science_281_5377_698_s_77	9685263	( A) Sec23-24p binding is localized to the COOH-terminal (membrane-proximal) 79 amino acids of the cytosolic domain of Bet1p, whereas Sar1p can bind to the 41 COOH-terminal amino acids of the cytosolic domain.	bind
1878	2	643	6	NULL	NULL	0	NULL	Sar1p	GP		bind					Bet1p	GP		41 COOH-terminal amino acids of the cytosolic domain		NULL		NULL	NULL	NULL	NULL	gw60_science_281_5377_698_s_77	9685263	( A) Sec23-24p binding is localized to the COOH-terminal (membrane-proximal) 79 amino acids of the cytosolic domain of Bet1p, whereas Sar1p can bind to the 41 COOH-terminal amino acids of the cytosolic domain.	bind
58210	1	644	5	NULL	NULL	0	NULL	trans-acting delta ribozyme	GP	engineered	bind					HBV target	Organism				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_21_4682_s_27	12409459	( A) Secondary structure of the engineered  trans-acting  delta ribozyme bound to the HBV target.	bind
58211	1	646	5	NULL	NULL	0	NULL	anti-RAS scFv	GP		bind					HRASG12V-GppNp antigen	GP				NULL		0	NULL	NULL	NULL	gw70_embo_22_5_1025_s_139	12606568	( A) Sensograms showing the binding of anti-RAS scFv with HRASG12V-GppNp antigen (immobilized  1500 RU).	bind
1879	1	646	6	NULL	NULL	0	NULL	anti-RAS scFv	GP		bind					HRASG12V-GppNp antigen	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_22_5_1025_s_139	12606568	( A) Sensograms showing the binding of anti-RAS scFv with HRASG12V-GppNp antigen (immobilized  1500 RU).	bind
58212	1	647	5	NULL	NULL	0	NULL	IGFBP-5	GP		bind					IGF-I	GP	biotinylated			NULL		0	NULL	NULL	NULL	gw60_embo_17_22_6558_s_62	9822601	( A) Sensograms showing the binding of IGFBP-5 to a sensor chip SA coated with 5 nM biotinylated IGF-I and IGF-II.	bind
58213	2	647	5	NULL	NULL	0	NULL	IGFBP-5	GP		bind					IGF-II	GP	biotinylated			NULL		0	NULL	NULL	NULL	gw60_embo_17_22_6558_s_62	9822601	( A) Sensograms showing the binding of IGFBP-5 to a sensor chip SA coated with 5 nM biotinylated IGF-I and IGF-II.	bind
1880	1	647	6	NULL	NULL	0	NULL	IGFBP-5 	GP		bind					IGF-I	GP	biotinylated			NULL		NULL	NULL	NULL	NULL	gw60_embo_17_22_6558_s_62	9822601	( A) Sensograms showing the binding of IGFBP-5 to a sensor chip SA coated with 5 nM biotinylated IGF-I and IGF-II.	bind
1881	2	647	6	NULL	NULL	0	NULL	IGFBP-5 	GP		bind					IGF-II	GP	biotinylated			NULL		NULL	NULL	NULL	NULL	gw60_embo_17_22_6558_s_62	9822601	( A) Sensograms showing the binding of IGFBP-5 to a sensor chip SA coated with 5 nM biotinylated IGF-I and IGF-II.	bind
58214	1	652	5	NULL	NULL	0	NULL	hairpin ribozyme	GP		bind					target RNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_pnas_98_1_130_s_92	11136250	( A) Sequence and secondary structure of the hairpin ribozyme (capital letters), bound to its target RNA (lowercase letters).	bind
1882	1	652	6	NULL	NULL	0	NULL	hairpin ribozyme	NucleicAcid		bind					target RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_1_130_s_92	11136250	( A) Sequence and secondary structure of the hairpin ribozyme (capital letters), bound to its target RNA (lowercase letters).	bind
58215	1	658	5	NULL	NULL	0	NULL	SIP1	GP		bind			FS		alpha4-integrin	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5073_s_137	10487759	( A) SIP1FS and SIP1CZF bind to the alpha4-integrin (alpha4I) promoter.	bind
58216	2	658	5	NULL	NULL	0	NULL	SIP1	GP		bind			CZF		alpha4-integrin	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5073_s_137	10487759	( A) SIP1FS and SIP1CZF bind to the alpha4-integrin (alpha4I) promoter.	bind
58217	3	658	5	NULL	NULL	0	NULL	alpha4-integrin	GP		is					alpha4I	GP				NULL		0	NULL	NULL	NULL	gw60_embo_18_18_5073_s_137	10487759	( A) SIP1FS and SIP1CZF bind to the alpha4-integrin (alpha4I) promoter.	bind
1883	1	658	6	NULL	NULL	0	NULL	SIP1	GP		bind			FS		alpha4-integrin 	GP			Promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5073_s_137	10487759	( A) SIP1FS and SIP1CZF bind to the alpha4-integrin (alpha4I) promoter.	bind
1884	2	658	6	NULL	NULL	0	NULL	SIP1	GP		bind			CZF		alpha4-integrin 	GP			Promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5073_s_137	10487759	( A) SIP1FS and SIP1CZF bind to the alpha4-integrin (alpha4I) promoter.	bind
51839	3	658	6	NULL	NULL	0	NULL	alpha4I	GP		is					alpha4-integrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5073_s_137	10487759	( A) SIP1FS and SIP1CZF bind to the alpha4-integrin (alpha4I) promoter.	bind
58218	1	659	5	NULL	NULL	0	NULL	SipA	GP		does not bind		directly			T-plastin	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_96_18_10176_s_119	10468582	( A) SipA does not bind to T-plastin directly.	bind
1885	1	659	6	NULL	NULL	0	NULL	SipA	GP		does not bind		directly			T-plastin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_18_10176_s_119	10468582	( A) SipA does not bind to T-plastin directly.	bind
58219	1	660	5	NULL	NULL	0	NULL	SKAP55	GP		bind			SH3 domain		FYB	GP				NULL	COS cells	0	NULL	NULL	NULL	gw60_pnas_95_15_8779_s_139	9671755	( A) SKAP55 and SKAP55R SH3 domains bind to FYB in COS cells.	bind
58220	2	660	5	NULL	NULL	0	NULL	SKAP55R	GP		bind			SH3 domain		FYB	GP				NULL	COS cells	NULL	NULL	NULL	NULL	gw60_pnas_95_15_8779_s_139	9671755	( A) SKAP55 and SKAP55R SH3 domains bind to FYB in COS cells.	bind
1886	1	660	6	NULL	NULL	0	NULL	SKAP55	GP		bind			SH3 domains		FYB	GP				NULL	COS cells	NULL	NULL	NULL	NULL	gw60_pnas_95_15_8779_s_139	9671755	( A) SKAP55 and SKAP55R SH3 domains bind to FYB in COS cells.	bind
1887	2	660	6	NULL	NULL	0	NULL	SKAP55R 	GP		bind			SH3 domains		FYB	GP				NULL	COS cells	NULL	NULL	NULL	NULL	gw60_pnas_95_15_8779_s_139	9671755	( A) SKAP55 and SKAP55R SH3 domains bind to FYB in COS cells.	bind
58221	1	661	5	NULL	NULL	0	NULL	Smad3	GP		bind			MH1 domain		HEF1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_24_6759_s_115	11118211	( A) Smad3 binds to HEF1 via both Smad3N (MH1) and Smad3C (MH2) domains, but only the N-terminal domain induces the degradation of HEF1.	bind
58222	2	661	5	NULL	NULL	0	NULL	Smad3	GP		bind			MH2 domain		HEF1	GP				NULL		0	NULL	NULL	NULL	gw60_embo_19_24_6759_s_115	11118211	( A) Smad3 binds to HEF1 via both Smad3N (MH1) and Smad3C (MH2) domains, but only the N-terminal domain induces the degradation of HEF1.	bind
58223	3	661	5	NULL	NULL	0	NULL	statement 1	Process		induces					HEF1	GP	degradation of			NULL		0	NULL	NULL	NULL	gw60_embo_19_24_6759_s_115	11118211	( A) Smad3 binds to HEF1 via both Smad3N (MH1) and Smad3C (MH2) domains, but only the N-terminal domain induces the degradation of HEF1.	bind
58224	4	661	5	NULL	NULL	0	NULL	MH1 domain			is					Smad3N					NULL		0	NULL	NULL	NULL	gw60_embo_19_24_6759_s_115	11118211	( A) Smad3 binds to HEF1 via both Smad3N (MH1) and Smad3C (MH2) domains, but only the N-terminal domain induces the degradation of HEF1.	bind
58225	5	661	5	NULL	NULL	0	NULL	MH2 domain			is					Smad3C					NULL		0	NULL	NULL	NULL	gw60_embo_19_24_6759_s_115	11118211	( A) Smad3 binds to HEF1 via both Smad3N (MH1) and Smad3C (MH2) domains, but only the N-terminal domain induces the degradation of HEF1.	bind
1888	1	661	6	NULL	NULL	0	NULL	Smad3	GP		bind			Smad3N		HEF1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_24_6759_s_115	11118211	( A) Smad3 binds to HEF1 via both Smad3N (MH1) and Smad3C (MH2) domains, but only the N-terminal domain induces the degradation of HEF1.	bind
1889	2	661	6	NULL	NULL	0	NULL	Smad3	GP		bind			Smad3C domain		HEF1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_24_6759_s_115	11118211	( A) Smad3 binds to HEF1 via both Smad3N (MH1) and Smad3C (MH2) domains, but only the N-terminal domain induces the degradation of HEF1.	bind
1890	3	661	6	NULL	NULL	0	NULL	Smad3	GP		induces			N-terminal domain		HEF1	GP	degradation of 			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_24_6759_s_115	11118211	( A) Smad3 binds to HEF1 via both Smad3N (MH1) and Smad3C (MH2) domains, but only the N-terminal domain induces the degradation of HEF1.	bind
51937	4	661	6	NULL	NULL	0	NULL	Smad3N	GP		is					MH1 domain	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_24_6759_s_115	11118211	( A) Smad3 binds to HEF1 via both Smad3N (MH1) and Smad3C (MH2) domains, but only the N-terminal domain induces the degradation of HEF1.	bind
51938	5	661	6	NULL	NULL	0	NULL	 Smad3C	GP		is					MH2 domain	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_24_6759_s_115	11118211	( A) Smad3 binds to HEF1 via both Smad3N (MH1) and Smad3C (MH2) domains, but only the N-terminal domain induces the degradation of HEF1.	bind
58226	1	662	5	NULL	NULL	0	NULL	SnoN	GP		interacts with					Smad4	GP				NULL		0	NULL	NULL	NULL	gw60_science_286_5440_771_s_55	10531062	( A) SnoN binds to the SBE through interaction with Smad4.	bind
58227	2	662	5	NULL	NULL	0	NULL	statement 1	Process		bind									SBE	NULL		0	NULL	NULL	NULL	gw60_science_286_5440_771_s_55	10531062	( A) SnoN binds to the SBE through interaction with Smad4.	bind
1891	1	662	6	NULL	NULL	0	NULL	SnoN	GP		interacts 					Smad4	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5440_771_s_55	10531062	( A) SnoN binds to the SBE through interaction with Smad4.	bind
1892	2	662	6	NULL	NULL	0	NULL	Statement 1	Process		bind						NucleicAcid			SBE	NULL		NULL	NULL	NULL	NULL	gw60_science_286_5440_771_s_55	10531062	( A) SnoN binds to the SBE through interaction with Smad4.	bind
58228	1	663	5	NULL	NULL	0	NULL	SOCS2	GP		bind					elongin C	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_103_20_7637_s_54	16675548	( A) SOCS2 binds elongin C (electrostatic surface shown) in a hydrophobic interface of   2,200  Ang 2 (for clarity, elongin B is not shown).	bind
1893	1	663	6	NULL	NULL	0	NULL	SOCS2	GP		bind					elongin C	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_20_7637_s_54	16675548	( A) SOCS2 binds elongin C (electrostatic surface shown) in a hydrophobic interface of   2,200  Ang 2 (for clarity, elongin B is not shown).	bind
58229	1	665	5	NULL	NULL	0	NULL	HKa	GP		bind		specifically			tropomyosin	GP	purified			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_19_12224_s_154	12196635	( A) Specific binding of HKa to purified tropomyosin.	bind
1894	1	665	6	NULL	NULL	0	NULL	HKa	GP		bind		specifically			tropomyosin	GP	purified			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_19_12224_s_154	12196635	( A) Specific binding of HKa to purified tropomyosin.	bind
58230	1	666	5	NULL	NULL	0	NULL	CTCF	GP		bind									Meg1 repeat	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_5_1398_s_127	12595547	( A) Specific competition for CTCF binding to the  Meg1 repeat was seen for the canonical CTCF- binding sequence of the chicken beta -globin FII (as shown in F), but not for the transcription factor recognition sequences of SP1 and AP1 (as shown in S and A) and vice versa.	bind
58231	2	666	5	NULL	NULL	0	NULL	CTCF	GP		bind					beta -globin FII	GP	chicken	CTCF- binding sequence		NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_5_1398_s_127	12595547	( A) Specific competition for CTCF binding to the  Meg1 repeat was seen for the canonical CTCF- binding sequence of the chicken beta -globin FII (as shown in F), but not for the transcription factor recognition sequences of SP1 and AP1 (as shown in S and A) and vice versa.	bind
58232	3	666	5	NULL	NULL	0	NULL	statement 1	Process		competes with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_5_1398_s_127	12595547	( A) Specific competition for CTCF binding to the  Meg1 repeat was seen for the canonical CTCF- binding sequence of the chicken beta -globin FII (as shown in F), but not for the transcription factor recognition sequences of SP1 and AP1 (as shown in S and A) and vice versa.	bind
58234	4	666	5	NULL	NULL	0	NULL	SP1	GP		does not compete with					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_5_1398_s_127	12595547	( A) Specific competition for CTCF binding to the  Meg1 repeat was seen for the canonical CTCF- binding sequence of the chicken beta -globin FII (as shown in F), but not for the transcription factor recognition sequences of SP1 and AP1 (as shown in S and A) and vice versa.	bind
58235	5	666	5	NULL	NULL	0	NULL	AP1	GP		does not compete with					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_5_1398_s_127	12595547	( A) Specific competition for CTCF binding to the  Meg1 repeat was seen for the canonical CTCF- binding sequence of the chicken beta -globin FII (as shown in F), but not for the transcription factor recognition sequences of SP1 and AP1 (as shown in S and A) and vice versa.	bind
2158	1	666	6	NULL	NULL	0	NULL	beta -globin FII	GP	chicken	bind				CTCF- binding sequence	CTCF 	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_5_1398_s_127	12595547	( A) Specific competition for CTCF binding to the  Meg1 repeat was seen for the canonical CTCF- binding sequence of the chicken beta -globin FII (as shown in F), but not for the transcription factor recognition sequences of SP1 and AP1 (as shown in S and A) and vice versa.	bind
2159	2	666	6	NULL	NULL	0	NULL	CTCF	GP		bind						NucleicAcid			Meg1 repeat	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_5_1398_s_127	12595547	( A) Specific competition for CTCF binding to the  Meg1 repeat was seen for the canonical CTCF- binding sequence of the chicken beta -globin FII (as shown in F), but not for the transcription factor recognition sequences of SP1 and AP1 (as shown in S and A) and vice versa.	bind
2160	3	666	6	NULL	NULL	0	NULL	statement 1	Process		competes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_5_1398_s_127	12595547	( A) Specific competition for CTCF binding to the  Meg1 repeat was seen for the canonical CTCF- binding sequence of the chicken beta -globin FII (as shown in F), but not for the transcription factor recognition sequences of SP1 and AP1 (as shown in S and A) and vice versa.	bind
2192	4	666	6	NULL	NULL	0	NULL	Sp1	GP		does not compete					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_5_1398_s_127	12595547	( A) Specific competition for CTCF binding to the  Meg1 repeat was seen for the canonical CTCF- binding sequence of the chicken beta -globin FII (as shown in F), but not for the transcription factor recognition sequences of SP1 and AP1 (as shown in S and A) and vice versa.	bind
2193	5	666	6	NULL	NULL	0	NULL	Ap1	GP		does not compete					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_5_1398_s_127	12595547	( A) Specific competition for CTCF binding to the  Meg1 repeat was seen for the canonical CTCF- binding sequence of the chicken beta -globin FII (as shown in F), but not for the transcription factor recognition sequences of SP1 and AP1 (as shown in S and A) and vice versa.	bind
58236	1	667	5	NULL	NULL	0	NULL	sperm	Cell		release					MSP	GP				NULL		0	NULL	NULL	NULL	gw60_genesdev_17_2_187_s_257	12533508	( a) Sperm release MSP, which binds to VAB-1 and another receptor(s) on oocytes and sheath cells.	bind
58237	2	667	5	NULL	NULL	0	NULL	MSP	GP		bind					VAB-1	GP				NULL	oocytes	0	NULL	NULL	NULL	gw60_genesdev_17_2_187_s_257	12533508	( a) Sperm release MSP, which binds to VAB-1 and another receptor(s) on oocytes and sheath cells.	bind
58238	3	667	5	NULL	NULL	0	NULL	MSP	GP		bind					VAB-1	GP				NULL	sheath cells	0	NULL	NULL	NULL	gw60_genesdev_17_2_187_s_257	12533508	( a) Sperm release MSP, which binds to VAB-1 and another receptor(s) on oocytes and sheath cells.	bind
1914	1	667	6	NULL	NULL	0	NULL	sperm	Cell		release					MSP	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_2_187_s_257	12533508	( a) Sperm release MSP, which binds to VAB-1 and another receptor(s) on oocytes and sheath cells.	bind
1915	2	667	6	NULL	NULL	0	NULL	MSP	GP		bind					VAB-1	GP				NULL	oocytes	NULL	NULL	NULL	NULL	gw60_genesdev_17_2_187_s_257	12533508	( a) Sperm release MSP, which binds to VAB-1 and another receptor(s) on oocytes and sheath cells.	bind
1916	3	667	6	NULL	NULL	0	NULL	MSP	GP		bind					receptor	GP				NULL	oocytes 	NULL	NULL	NULL	NULL	gw60_genesdev_17_2_187_s_257	12533508	( a) Sperm release MSP, which binds to VAB-1 and another receptor(s) on oocytes and sheath cells.	bind
51967	4	667	6	NULL	NULL	0	NULL	MSP	GP		bind					VAB-1	GP				NULL	sheath cells	NULL	NULL	NULL	NULL	gw60_genesdev_17_2_187_s_257	12533508	( a) Sperm release MSP, which binds to VAB-1 and another receptor(s) on oocytes and sheath cells.	bind
51968	6	667	6	NULL	NULL	0	NULL	MSP	GP		bind					receptor	GP				NULL	sheath cells	NULL	NULL	NULL	NULL	gw60_genesdev_17_2_187_s_257	12533508	( a) Sperm release MSP, which binds to VAB-1 and another receptor(s) on oocytes and sheath cells.	bind
58239	1	669	5	NULL	NULL	0	NULL	lipid layers	Chemical		contains					PIP2	Chemical				NULL		0	NULL	NULL	NULL	gw70_embo_24_14_2556_s_150	15961997	( A) SPR sensograms showing the binding of the individual PDZ domains of syntenin-2 to  10% PIP2-containing lipid layers.	bind
58240	2	669	5	NULL	NULL	0	NULL	syntenin-2	GP		bind			PDZ domain		statement 1	Chemical				NULL		0	NULL	NULL	NULL	gw70_embo_24_14_2556_s_150	15961997	( A) SPR sensograms showing the binding of the individual PDZ domains of syntenin-2 to  10% PIP2-containing lipid layers.	bind
1917	2	669	6	NULL	NULL	0	NULL	syntenin-2	GP		bind			individual PDZ domains		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_14_2556_s_150	15961997	( A) SPR sensograms showing the binding of the individual PDZ domains of syntenin-2 to  10% PIP2-containing lipid layers.	bind
51969	1	669	6	NULL	NULL	0	NULL	lipid layers	CellComponent		contain					PIP2	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_14_2556_s_150	15961997	( A) SPR sensograms showing the binding of the individual PDZ domains of syntenin-2 to  10% PIP2-containing lipid layers.	bind
58241	1	672	5	NULL	NULL	0	NULL	uPA	GP		bind			beta-hairpin in GFD		uPAR	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_9_1655_s_132	15861141	( A) Stereo views of the key residues by which AE147 (blue) and the beta-hairpin in GFD of uPA (red) bind to uPAR in our crystal structure and in a GFD uPAR  model, respectively.	bind
1918	1	672	6	NULL	NULL	0	NULL	uPA	GP		bind			AE147		uPAR	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_9_1655_s_132	15861141	( A) Stereo views of the key residues by which AE147 (blue) and the beta-hairpin in GFD of uPA (red) bind to uPAR in our crystal structure and in a GFD uPAR  model, respectively.	bind
1919	2	672	6	NULL	NULL	0	NULL	uPA	GP		bind			beta-hairpin in GFD		uPAR	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_9_1655_s_132	15861141	( A) Stereo views of the key residues by which AE147 (blue) and the beta-hairpin in GFD of uPA (red) bind to uPAR in our crystal structure and in a GFD uPAR  model, respectively.	bind
58242	1	673	5	NULL	NULL	0	NULL	Npl4	GP		bind			NZF		Ub	GP				NULL		0	NULL	NULL	NULL	gw70_embo_23_7_1411_s_55	15029239	( A) Stereoview of Npl4 NZF (ribbon) bound to Ub (surface).	bind
1920	1	673	6	NULL	NULL	0	NULL	Npl4	GP		bind			NZF		Ub	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1411_s_55	15029239	( A) Stereoview of Npl4 NZF (ribbon) bound to Ub (surface).	bind
58243	1	678	5	NULL	NULL	0	NULL	Sos peptide (PPPVPPRRR)	AminoAcid	wild-type	bind					Crk	GP		SH3 domain		NULL		0	NULL	NULL	NULL	gw60_science_282_5396_2088_s_106	9851931	( A) Structure of wild-type Sos peptide (PPPVPPRRR) bound to Crk SH3 domain ( 20).	bind
1921	1	678	6	NULL	NULL	0	NULL	Sos peptide	GP	wild type	bind			PPPVPPRRR		Crk	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_science_282_5396_2088_s_106	9851931	( A) Structure of wild-type Sos peptide (PPPVPPRRR) bound to Crk SH3 domain ( 20).	bind
58244	1	680	5	NULL	NULL	0	NULL	Sum1	GP		bind					HML-E	GP				NULL	in vitro	0	NULL	NULL	NULL	gw70_genesdev_19_15_1811_s_149	16077008	( A) Sum1 bound in vitro to  HML-E, but not the  INO1 promoter region.	bind
58245	2	680	5	NULL	NULL	0	NULL	Sum1	GP		does not bind					INO1	GP			promoter	NULL		0	NULL	NULL	NULL	gw70_genesdev_19_15_1811_s_149	16077008	( A) Sum1 bound in vitro to  HML-E, but not the  INO1 promoter region.	bind
1922	1	680	6	NULL	NULL	0	NULL	Sum1	GP		bind					HML-E	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_genesdev_19_15_1811_s_149	16077008	( A) Sum1 bound in vitro to  HML-E, but not the  INO1 promoter region.	bind
1923	2	680	6	NULL	NULL	0	NULL	Sum1	GP		does not bind					INO1	GP			Promoter	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_15_1811_s_149	16077008	( A) Sum1 bound in vitro to  HML-E, but not the  INO1 promoter region.	bind
58246	1	690	5	NULL	NULL	0	NULL	SWI/SNF	GP		bind		efficiently			H2ABbd nucleosomes	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_19_3815_s_94	15372075	( A) SWI/SNF efficiently binds H2ABbd nucleosomes.	bind
1965	1	690	6	NULL	NULL	0	NULL	SWI/SNF	GP		bind		efficiently			H2ABbd nucleosomes	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_19_3815_s_94	15372075	( A) SWI/SNF efficiently binds H2ABbd nucleosomes.	bind
58247	1	691	5	NULL	NULL	0	NULL	TFIIB	GP		bind					GAPDH	GP				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_4_717_s_157	16332727	( A) TFIIB binding to GAPDH.	bind
1966	1	691	6	NULL	NULL	0	NULL	TFIIB	GP		bind					GAPDH	GP				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_4_717_s_157	16332727	( A) TFIIB binding to GAPDH.	bind
58248	1	693	5	NULL	NULL	0	NULL	TGF-beta1	GP		bind					ALK1	GP				NULL	HUVEC	0	NULL	NULL	NULL	gw60_pnas_97_6_2626_s_172	10716993	( A) TGF-beta1 binds to ALK1 as well as ALK5 (TbetaR-I) in HUVEC.	bind
58249	2	693	5	NULL	NULL	0	NULL	TGF-beta1	GP		bind					ALK5	GP				NULL	HUVEC	0	NULL	NULL	NULL	gw60_pnas_97_6_2626_s_172	10716993	( A) TGF-beta1 binds to ALK1 as well as ALK5 (TbetaR-I) in HUVEC.	bind
58250	3	693	5	NULL	NULL	0	NULL	ALK5	GP		is					TbetaR-I	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_97_6_2626_s_172	10716993	( A) TGF-beta1 binds to ALK1 as well as ALK5 (TbetaR-I) in HUVEC.	bind
1967	1	693	6	NULL	NULL	0	NULL	TGF-beta1	GP		bind					ALK1	GP				NULL	HUVEC	NULL	NULL	NULL	NULL	gw60_pnas_97_6_2626_s_172	10716993	( A) TGF-beta1 binds to ALK1 as well as ALK5 (TbetaR-I) in HUVEC.	bind
1968	2	693	6	NULL	NULL	0	NULL	TGF-beta1	GP		bind					ALK5	GP				NULL	HUVEC	NULL	NULL	NULL	NULL	gw60_pnas_97_6_2626_s_172	10716993	( A) TGF-beta1 binds to ALK1 as well as ALK5 (TbetaR-I) in HUVEC.	bind
58251	1	695	5	NULL	NULL	0	NULL	GST-eIF5	GP		bind					eIF2	GP	native;;purified			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_18_6_1673_s_100	10075937	( A) The 7A mutation in GST-eIF5 impairs its binding to purified native eIF2 and eIF3  in vitro.	bind
58252	2	695	5	NULL	NULL	0	NULL	GST-eIF5	GP	mutant	impairs					statement 1	Process				NULL	in vitro	0	NULL	NULL	NULL	gw60_embo_18_6_1673_s_100	10075937	( A) The 7A mutation in GST-eIF5 impairs its binding to purified native eIF2 and eIF3  in vitro.	bind
58253	3	695	5	NULL	NULL	0	NULL	GST-eIF5	GP		bind					eIF3	GP	native;;purified			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_18_6_1673_s_100	10075937	( A) The 7A mutation in GST-eIF5 impairs its binding to purified native eIF2 and eIF3  in vitro.	bind
58254	4	695	5	NULL	NULL	0	NULL	GST-eIF5	GP	mutant	impairs					statement 3	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_18_6_1673_s_100	10075937	( A) The 7A mutation in GST-eIF5 impairs its binding to purified native eIF2 and eIF3  in vitro.	bind
1969	1	695	6	NULL	NULL	0	NULL	GST-eIF5	GP		bind					eIF2	GP	purified			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_18_6_1673_s_100	10075937	( A) The 7A mutation in GST-eIF5 impairs its binding to purified native eIF2 and eIF3  in vitro.	bind
1970	2	695	6	NULL	NULL	0	NULL	GST-eIF5	GP		bind					eIF3	GP	purified			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_18_6_1673_s_100	10075937	( A) The 7A mutation in GST-eIF5 impairs its binding to purified native eIF2 and eIF3  in vitro.	bind
1971	3	695	6	NULL	NULL	0	NULL	GST-eIF5	GP		impairs			mutant 7A		Statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_6_1673_s_100	10075937	( A) The 7A mutation in GST-eIF5 impairs its binding to purified native eIF2 and eIF3  in vitro.	bind
1972	4	695	6	NULL	NULL	0	NULL	GST-eIF5	GP		impairs			mutant 7A		Statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_6_1673_s_100	10075937	( A) The 7A mutation in GST-eIF5 impairs its binding to purified native eIF2 and eIF3  in vitro.	bind
58255	1	696	5	NULL	NULL	0	NULL	ADP-ribose molecule	Chemical		bind					Af1521	GP		macro domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_11_1911_s_111	15902274	( A) The ADP-ribose molecule binds the Af1521  macro domain in an L-shaped cleft.	bind
1973	1	696	6	NULL	NULL	0	NULL	ADP-ribose molecule	Chemical		bind					Af1521	GP		macro domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_11_1911_s_111	15902274	( A) The ADP-ribose molecule binds the Af1521  macro domain in an L-shaped cleft.	bind
58256	1	698	5	NULL	NULL	0	NULL	synaptosome	CellComponent		contains					AMPA receptor	GP		GluR2/3 subunit		NULL		0	NULL	NULL	NULL	gw70_embo_22_3_558_s_164	12554656	( A) The AMPA receptor subunits GluR2/3 and GluR1, the GluR2/3 binding partner GRIP,  the NMDA receptor subunit NR1, the plasma membrane marker Na+/K+ ATPase and the synaptic vesicle protein synaptophysin are all clearly detectable  in the crude synaptosome fraction (P2).	bind
58257	2	698	5	NULL	NULL	0	NULL	synaptosome	CellComponent		contains					AMPA receptor	GP		GluR1 subunit		NULL		0	NULL	NULL	NULL	gw70_embo_22_3_558_s_164	12554656	( A) The AMPA receptor subunits GluR2/3 and GluR1, the GluR2/3 binding partner GRIP,  the NMDA receptor subunit NR1, the plasma membrane marker Na+/K+ ATPase and the synaptic vesicle protein synaptophysin are all clearly detectable  in the crude synaptosome fraction (P2).	bind
58258	3	698	5	NULL	NULL	0	NULL	GRIP	GP		bind					GluR2/3	GP				NULL		0	NULL	NULL	NULL	gw70_embo_22_3_558_s_164	12554656	( A) The AMPA receptor subunits GluR2/3 and GluR1, the GluR2/3 binding partner GRIP,  the NMDA receptor subunit NR1, the plasma membrane marker Na+/K+ ATPase and the synaptic vesicle protein synaptophysin are all clearly detectable  in the crude synaptosome fraction (P2).	bind
58259	4	698	5	NULL	NULL	0	NULL	synaptosome	CellComponent		contains					GRIP	GP				NULL		0	NULL	NULL	NULL	gw70_embo_22_3_558_s_164	12554656	( A) The AMPA receptor subunits GluR2/3 and GluR1, the GluR2/3 binding partner GRIP,  the NMDA receptor subunit NR1, the plasma membrane marker Na+/K+ ATPase and the synaptic vesicle protein synaptophysin are all clearly detectable  in the crude synaptosome fraction (P2).	bind
58260	5	698	5	NULL	NULL	0	NULL	synaptosome	CellComponent		contains					NMDA receptor	GP		NR1 subunit		NULL		0	NULL	NULL	NULL	gw70_embo_22_3_558_s_164	12554656	( A) The AMPA receptor subunits GluR2/3 and GluR1, the GluR2/3 binding partner GRIP,  the NMDA receptor subunit NR1, the plasma membrane marker Na+/K+ ATPase and the synaptic vesicle protein synaptophysin are all clearly detectable  in the crude synaptosome fraction (P2).	bind
58261	6	698	5	NULL	NULL	0	NULL	synaptosome	CellComponent		contains					Na+/K+ ATPase	GP				NULL		0	NULL	NULL	NULL	gw70_embo_22_3_558_s_164	12554656	( A) The AMPA receptor subunits GluR2/3 and GluR1, the GluR2/3 binding partner GRIP,  the NMDA receptor subunit NR1, the plasma membrane marker Na+/K+ ATPase and the synaptic vesicle protein synaptophysin are all clearly detectable  in the crude synaptosome fraction (P2).	bind
58262	7	698	5	NULL	NULL	0	NULL	synaptosome	CellComponent		contains					synaptophysin	GP				NULL		0	NULL	NULL	NULL	gw70_embo_22_3_558_s_164	12554656	( A) The AMPA receptor subunits GluR2/3 and GluR1, the GluR2/3 binding partner GRIP,  the NMDA receptor subunit NR1, the plasma membrane marker Na+/K+ ATPase and the synaptic vesicle protein synaptophysin are all clearly detectable  in the crude synaptosome fraction (P2).	bind
58263	8	698	5	NULL	NULL	0	NULL	synaptophysin	GP		is a type of					synaptic vesicle protein 	GP				NULL		0	NULL	NULL	NULL	gw70_embo_22_3_558_s_164	12554656	( A) The AMPA receptor subunits GluR2/3 and GluR1, the GluR2/3 binding partner GRIP,  the NMDA receptor subunit NR1, the plasma membrane marker Na+/K+ ATPase and the synaptic vesicle protein synaptophysin are all clearly detectable  in the crude synaptosome fraction (P2).	bind
58264	9	698	5	NULL	NULL	0	NULL	Na+/K+ ATPase	GP		is a type of					plasma membrane marker	GP				NULL		0	NULL	NULL	NULL	gw70_embo_22_3_558_s_164	12554656	( A) The AMPA receptor subunits GluR2/3 and GluR1, the GluR2/3 binding partner GRIP,  the NMDA receptor subunit NR1, the plasma membrane marker Na+/K+ ATPase and the synaptic vesicle protein synaptophysin are all clearly detectable  in the crude synaptosome fraction (P2).	bind
58265	1	702	5	NULL	NULL	0	NULL	holo-Tf	GP		bind					Tf	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_102_34_12095_s_142	16103367	( A) The binding of holo-Tf to TfR has no effect on GA-induced apoptosis.	bind
58266	2	702	5	NULL	NULL	0	NULL	apoptosis	Process		is induced by					GA	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_34_12095_s_142	16103367	( A) The binding of holo-Tf to TfR has no effect on GA-induced apoptosis.	bind
58267	3	702	5	NULL	NULL	0	NULL	statement 1	Process		does not effect					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_102_34_12095_s_142	16103367	( A) The binding of holo-Tf to TfR has no effect on GA-induced apoptosis.	bind
1974	1	702	6	NULL	NULL	0	NULL	holo-Tf	GP		bind					TfR	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_34_12095_s_142	16103367	( A) The binding of holo-Tf to TfR has no effect on GA-induced apoptosis.	bind
1975	3	702	6	NULL	NULL	0	NULL	Statement 1	Process		has no effect on					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_34_12095_s_142	16103367	( A) The binding of holo-Tf to TfR has no effect on GA-induced apoptosis.	bind
51970	2	702	6	NULL	NULL	0	NULL	GA	Chemical		induce					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_34_12095_s_142	16103367	( A) The binding of holo-Tf to TfR has no effect on GA-induced apoptosis.	bind
58268	1	703	5	NULL	NULL	0	NULL	JIP-1	GP		bind					HPK1	GP				NULL		0	NULL	NULL	NULL	gw60_science_281_5383_1671_s_77	9733513	( A) The binding of JIP-1 to HPK1, MLK3, DLK, and MKK7 is independent of JNK.	bind
58269	2	703	5	NULL	NULL	0	NULL	statement 1	Process		is independent of					JNK	GP				NULL		0	NULL	NULL	NULL	gw60_science_281_5383_1671_s_77	9733513	( A) The binding of JIP-1 to HPK1, MLK3, DLK, and MKK7 is independent of JNK.	bind
58270	3	703	5	NULL	NULL	0	NULL	JIP-1	GP		bind					MLK3	GP				NULL		0	NULL	NULL	NULL	gw60_science_281_5383_1671_s_77	9733513	( A) The binding of JIP-1 to HPK1, MLK3, DLK, and MKK7 is independent of JNK.	bind
58271	4	703	5	NULL	NULL	0	NULL	statement 3	Process		is independent of					JNK	GP				NULL		0	NULL	NULL	NULL	gw60_science_281_5383_1671_s_77	9733513	( A) The binding of JIP-1 to HPK1, MLK3, DLK, and MKK7 is independent of JNK.	bind
58272	5	703	5	NULL	NULL	0	NULL	JIP-1	GP		bind					DLK	GP				NULL		0	NULL	NULL	NULL	gw60_science_281_5383_1671_s_77	9733513	( A) The binding of JIP-1 to HPK1, MLK3, DLK, and MKK7 is independent of JNK.	bind
58273	6	703	5	NULL	NULL	0	NULL	statement 5	Process		is independent of					JNK	GP				NULL		0	NULL	NULL	NULL	gw60_science_281_5383_1671_s_77	9733513	( A) The binding of JIP-1 to HPK1, MLK3, DLK, and MKK7 is independent of JNK.	bind
58274	7	703	5	NULL	NULL	0	NULL	JIP-1	GP		bind					MKK7	GP				NULL		0	NULL	NULL	NULL	gw60_science_281_5383_1671_s_77	9733513	( A) The binding of JIP-1 to HPK1, MLK3, DLK, and MKK7 is independent of JNK.	bind
58275	8	703	5	NULL	NULL	0	NULL	statement 7	Process		is independent of					JNK	GP				NULL		0	NULL	NULL	NULL	gw60_science_281_5383_1671_s_77	9733513	( A) The binding of JIP-1 to HPK1, MLK3, DLK, and MKK7 is independent of JNK.	bind
1976	1	703	6	NULL	NULL	0	NULL	JIP-1	GP		bind					HPK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5383_1671_s_77	9733513	( A) The binding of JIP-1 to HPK1, MLK3, DLK, and MKK7 is independent of JNK.	bind
1977	2	703	6	NULL	NULL	0	NULL	JIP-1	GP		bind					MLK3	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5383_1671_s_77	9733513	( A) The binding of JIP-1 to HPK1, MLK3, DLK, and MKK7 is independent of JNK.	bind
1978	3	703	6	NULL	NULL	0	NULL	JIP-1	GP		bind					DLK	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5383_1671_s_77	9733513	( A) The binding of JIP-1 to HPK1, MLK3, DLK, and MKK7 is independent of JNK.	bind
1979	4	703	6	NULL	NULL	0	NULL	JIP-1	GP		bind					MKK7	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5383_1671_s_77	9733513	( A) The binding of JIP-1 to HPK1, MLK3, DLK, and MKK7 is independent of JNK.	bind
2229	5	703	6	NULL	NULL	0	NULL	statement 1	Process		is independent of					JNK	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5383_1671_s_77	9733513	( A) The binding of JIP-1 to HPK1, MLK3, DLK, and MKK7 is independent of JNK.	bind
2230	6	703	6	NULL	NULL	0	NULL	statement 2	Process		is independent of					JNK	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5383_1671_s_77	9733513	( A) The binding of JIP-1 to HPK1, MLK3, DLK, and MKK7 is independent of JNK.	bind
2231	7	703	6	NULL	NULL	0	NULL	statement 3	Process		is independent of					JNK	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5383_1671_s_77	9733513	( A) The binding of JIP-1 to HPK1, MLK3, DLK, and MKK7 is independent of JNK.	bind
2232	8	703	6	NULL	NULL	0	NULL	statement 4	Process		is independent of					JNK	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5383_1671_s_77	9733513	( A) The binding of JIP-1 to HPK1, MLK3, DLK, and MKK7 is independent of JNK.	bind
58276	1	704	5	NULL	NULL	0	NULL	p38	GP	mutant	bind					MKP-5	GP				NULL		0	NULL	NULL	NULL	gw60_embo_20_3_466_s_316	11157753	( A) The binding of the mutant forms of p38 and ERK2 to MKP-5.	bind
58277	2	704	5	NULL	NULL	0	NULL	ERK2	GP	mutant	bind					MKP-5	GP				NULL		0	NULL	NULL	NULL	gw60_embo_20_3_466_s_316	11157753	( A) The binding of the mutant forms of p38 and ERK2 to MKP-5.	bind
1980	1	704	6	NULL	NULL	0	NULL	p38	GP	mutant	bind					MKP-5	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_466_s_316	11157753	( A) The binding of the mutant forms of p38 and ERK2 to MKP-5.	bind
1981	2	704	6	NULL	NULL	0	NULL	ERK2	GP	mutant	bind					MKP-5	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_466_s_316	11157753	( A) The binding of the mutant forms of p38 and ERK2 to MKP-5.	bind
58278	1	705	5	NULL	NULL	0	NULL	p38	GP	mutant	bind					RSK2	GP				NULL		0	NULL	NULL	NULL	gw60_embo_20_3_466_s_253	11157753	( A) The binding of the mutant forms of p38 and ERK2 to RSK2.	bind
58279	2	705	5	NULL	NULL	0	NULL	ERK2	GP	mutant	bind					RSK2	GP				NULL		0	NULL	NULL	NULL	gw60_embo_20_3_466_s_253	11157753	( A) The binding of the mutant forms of p38 and ERK2 to RSK2.	bind
1982	1	705	6	NULL	NULL	0	NULL	p38	GP	mutant	bind					RSK2	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_466_s_253	11157753	( A) The binding of the mutant forms of p38 and ERK2 to RSK2.	bind
1983	2	705	6	NULL	NULL	0	NULL	ERK2	GP	mutant	bind					RSK2	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_466_s_253	11157753	( A) The binding of the mutant forms of p38 and ERK2 to RSK2.	bind
58280	1	706	5	NULL	NULL	0	NULL	p38	GP	mutant	bind					MSK1	GP				NULL		0	NULL	NULL	NULL	gw60_embo_20_3_466_s_273	11157753	( A) The binding of the mutant forms of p38 to MSK1.	bind
1984	1	706	6	NULL	NULL	0	NULL	p38	GP	mutant	bind					MSK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_466_s_273	11157753	( A) The binding of the mutant forms of p38 to MSK1.	bind
58281	1	707	5	NULL	NULL	0	NULL	p38	GP	mutant	bind					MSK2	GP				NULL		0	NULL	NULL	NULL	gw60_embo_20_3_466_s_223	11157753	( A) The binding of the mutant forms of p38 to MSK2.	bind
1985	1	707	6	NULL	NULL	0	NULL	p38	GP	mutant	bind					MSK2	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_466_s_223	11157753	( A) The binding of the mutant forms of p38 to MSK2.	bind
58282	1	710	5	NULL	NULL	0	NULL	DlEC fragment	AminoAcid		bind		specifically			N-S2 cells	Cell				NULL		0	NULL	NULL	NULL	gw60_science_283_5398_91_s_91	9872749	( A) The DlEC fragment specifically binds to N-expressing S2 (N-S2) cells and does not bind to S2 cells alone.	bind
58283	2	710	5	NULL	NULL	0	NULL	DlEC fragment	AminoAcid		does not bind					S2 cells	Cell				NULL		0	NULL	NULL	NULL	gw60_science_283_5398_91_s_91	9872749	( A) The DlEC fragment specifically binds to N-expressing S2 (N-S2) cells and does not bind to S2 cells alone.	bind
58284	3	710	5	NULL	NULL	0	NULL	N-S2 cells	Cell		is					N-expressing S2 cells	Cell				NULL		0	NULL	NULL	NULL	gw60_science_283_5398_91_s_91	9872749	( A) The DlEC fragment specifically binds to N-expressing S2 (N-S2) cells and does not bind to S2 cells alone.	bind
1986	1	710	6	NULL	NULL	0	NULL		NucleicAcid		bind		specifically	DlEC fragment 		S2 (N-S2) cells	Cell	N-expressing			NULL		NULL	NULL	NULL	NULL	gw60_science_283_5398_91_s_91	9872749	( A) The DlEC fragment specifically binds to N-expressing S2 (N-S2) cells and does not bind to S2 cells alone.	bind
1987	2	710	6	NULL	NULL	0	NULL		NucleicAcid		does not bind			DlEC fragment 		S2 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_science_283_5398_91_s_91	9872749	( A) The DlEC fragment specifically binds to N-expressing S2 (N-S2) cells and does not bind to S2 cells alone.	bind
58285	1	712	5	NULL	NULL	0	NULL	eIF4E - eIF4G	GP		is					eIF4F core complex	GP				NULL		0	NULL	NULL	NULL	gw60_embo_19_16_4372_s_231	10944120	( A) The eIF4F core complex, eIF4E - eIF4G, binds tightly to capped mRNA. Dcp1 can bind eIF4G, but has no access to the cap.	bind
58286	2	712	5	NULL	NULL	0	NULL	eIF4E - eIF4G	GP		bind		tightly			mRNA	NucleicAcid	capped			NULL		0	NULL	NULL	NULL	gw60_embo_19_16_4372_s_231	10944120	( A) The eIF4F core complex, eIF4E - eIF4G, binds tightly to capped mRNA. Dcp1 can bind eIF4G, but has no access to the cap.	bind
58287	3	712	5	NULL	NULL	0	NULL	Dcp1	GP		bind					eIF4G	GP				NULL		0	NULL	NULL	NULL	gw60_embo_19_16_4372_s_231	10944120	( A) The eIF4F core complex, eIF4E - eIF4G, binds tightly to capped mRNA. Dcp1 can bind eIF4G, but has no access to the cap.	bind
58288	4	712	5	NULL	NULL	0	NULL	Dcp1	GP		does not bind					mRNA	NucleicAcid	capped			NULL		0	NULL	NULL	NULL	gw60_embo_19_16_4372_s_231	10944120	( A) The eIF4F core complex, eIF4E - eIF4G, binds tightly to capped mRNA. Dcp1 can bind eIF4G, but has no access to the cap.	bind
1988	1	712	6	NULL	NULL	0	NULL	eIF4F core complex	GP		constitute					eIF4E - eIF4G	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_16_4372_s_231	10944120	( A) The eIF4F core complex, eIF4E - eIF4G, binds tightly to capped mRNA. Dcp1 can bind eIF4G, but has no access to the cap.	bind
1989	2	712	6	NULL	NULL	0	NULL	 eIF4F core complex	GP		bind		tightly			mRNA	NucleicAcid	capped			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_16_4372_s_231	10944120	( A) The eIF4F core complex, eIF4E - eIF4G, binds tightly to capped mRNA. Dcp1 can bind eIF4G, but has no access to the cap.	bind
1990	3	712	6	NULL	NULL	0	NULL	Dcp1	GP		bind					eIF4G	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_16_4372_s_231	10944120	( A) The eIF4F core complex, eIF4E - eIF4G, binds tightly to capped mRNA. Dcp1 can bind eIF4G, but has no access to the cap.	bind
1991	4	712	6	NULL	NULL	0	NULL	Dcp1	GP		does not access					cap					NULL		NULL	NULL	NULL	NULL	gw60_embo_19_16_4372_s_231	10944120	( A) The eIF4F core complex, eIF4E - eIF4G, binds tightly to capped mRNA. Dcp1 can bind eIF4G, but has no access to the cap.	bind
58289	1	713	5	NULL	NULL	0	NULL	NHERF	GP		bind			PDZ domain		beta2 receptor	GP		tail		NULL		0	NULL	NULL	NULL	gw60_pnas_95_15_8496_s_107	9671706	( A) The first PDZ domain of NHERF binds well to the beta2 receptor tail, moderately to the P2Y1 receptor tail, and poorly to the P2Y2 receptor tail.	bind
58290	2	713	5	NULL	NULL	0	NULL	NHERF	GP		bind		moderately	PDZ domain		P2Y1 receptor	GP		tail		NULL		0	NULL	NULL	NULL	gw60_pnas_95_15_8496_s_107	9671706	( A) The first PDZ domain of NHERF binds well to the beta2 receptor tail, moderately to the P2Y1 receptor tail, and poorly to the P2Y2 receptor tail.	bind
58291	3	713	5	NULL	NULL	0	NULL	NHERF	GP		bind		poorly	PDZ domain		P2Y2 receptor	GP		tail		NULL		0	NULL	NULL	NULL	gw60_pnas_95_15_8496_s_107	9671706	( A) The first PDZ domain of NHERF binds well to the beta2 receptor tail, moderately to the P2Y1 receptor tail, and poorly to the P2Y2 receptor tail.	bind
1992	1	713	6	NULL	NULL	0	NULL	NHERF	GP		bind			first PDZ domain		beta2 receptor 	GP		tail		NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_15_8496_s_107	9671706	( A) The first PDZ domain of NHERF binds well to the beta2 receptor tail, moderately to the P2Y1 receptor tail, and poorly to the P2Y2 receptor tail.	bind
1993	2	713	6	NULL	NULL	0	NULL	NHERF	GP		bind		moderately	first PDZ domain		P2Y1 receptor	GP		tail		NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_15_8496_s_107	9671706	( A) The first PDZ domain of NHERF binds well to the beta2 receptor tail, moderately to the P2Y1 receptor tail, and poorly to the P2Y2 receptor tail.	bind
1994	3	713	6	NULL	NULL	0	NULL	NHERF	GP		bind		poorly	first PDZ domain		P2Y2 receptor 	GP		tail		NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_15_8496_s_107	9671706	( A) The first PDZ domain of NHERF binds well to the beta2 receptor tail, moderately to the P2Y1 receptor tail, and poorly to the P2Y2 receptor tail.	bind
58292	1	714	5	NULL	NULL	0	NULL	Loco	GP		interacts with			GoLoco motif		Galphai	GP	wild type			NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1341_s_64	15937221	( A) The GoLoco motif of Loco interacts with wild-type Galphai but not GalphaiQ205L, the GTP-bound form of Galphai, in yeast two-hybrid assays.	bind
58293	2	714	5	NULL	NULL	0	NULL	Loco	GP		does not interact with			GoLoco motif		Galphai	GP		Q205L		NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1341_s_64	15937221	( A) The GoLoco motif of Loco interacts with wild-type Galphai but not GalphaiQ205L, the GTP-bound form of Galphai, in yeast two-hybrid assays.	bind
1995	1	714	6	NULL	NULL	0	NULL	Loco	GP		interacts with			GoLoco motif		Galphai	GP	wild-type			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_11_1341_s_64	15937221	( A) The GoLoco motif of Loco interacts with wild-type Galphai but not GalphaiQ205L, the GTP-bound form of Galphai, in yeast two-hybrid assays.	bind
1996	2	714	6	NULL	NULL	0	NULL	Loco	GP		does not bind			GoLoco motif		Galphai	GP		Q205L		NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_11_1341_s_64	15937221	( A) The GoLoco motif of Loco interacts with wild-type Galphai but not GalphaiQ205L, the GTP-bound form of Galphai, in yeast two-hybrid assays.	bind
51971	3	714	6	NULL	NULL	0	NULL	GTP	Chemical		bind					Galphai	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_11_1341_s_64	15937221	( A) The GoLoco motif of Loco interacts with wild-type Galphai but not GalphaiQ205L, the GTP-bound form of Galphai, in yeast two-hybrid assays.	bind
58294	1	715	5	NULL	NULL	0	NULL	PACS-1	GP	HIS-tagged	bind			furin-binding region (115-255)		polycystin-2	GP		carboxy-terminal (741-871)		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_4_705_s_56	15692563	( A) The HIS-tagged furin-binding region of PACS-1 (amino acids 115 255) binds the carboxy-terminal  amino acids 741 871 of polycystin-2 fused to the MBP.	bind
58295	2	715	5	NULL	NULL	0	NULL	polycystin-2	GP		is a type of					MBP-fusion protein	GP				NULL		0	NULL	NULL	NULL	gw70_embo_24_4_705_s_56	15692563	( A) The HIS-tagged furin-binding region of PACS-1 (amino acids 115 255) binds the carboxy-terminal  amino acids 741 871 of polycystin-2 fused to the MBP.	bind
1997	1	715	6	NULL	NULL	0	NULL	PACS-1	GP	HIS-tagged 	bind			amino acids 115 255;;furin-binding region 		polycystin-2	GP		carboxy-terminal amino acids;; 741 871		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_4_705_s_56	15692563	( A) The HIS-tagged furin-binding region of PACS-1 (amino acids 115 255) binds the carboxy-terminal  amino acids 741 871 of polycystin-2 fused to the MBP.	bind
51973	2	715	6	NULL	NULL	0	NULL	polycystin-2	GP		is a type of					MBP fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_4_705_s_56	15692563	( A) The HIS-tagged furin-binding region of PACS-1 (amino acids 115 255) binds the carboxy-terminal  amino acids 741 871 of polycystin-2 fused to the MBP.	bind
58296	1	719	5	NULL	NULL	0	NULL	FITC cholera toxin	GP		bind					GM1	GP				NULL	surface of a stage 3 neuron	0	NULL	NULL	NULL	gw60_embo_18_7_1761_s_45	10202140	( A) The labeling corresponding to the FITC cholera toxin bound to GM1 in the surface of a stage 3 neuron is shown on the left panel (GM1).	bind
1998	1	719	6	NULL	NULL	0	NULL	cholera toxin	Chemical		bind					GM1	GP				NULL	surface of a stage 3 neuron	NULL	NULL	NULL	NULL	gw60_embo_18_7_1761_s_45	10202140	( A) The labeling corresponding to the FITC cholera toxin bound to GM1 in the surface of a stage 3 neuron is shown on the left panel (GM1).	bind
58297	1	722	5	NULL	NULL	0	NULL	pheromone	GP		is a type of					mating factor	GP				NULL		0	NULL	NULL	NULL	gw70_annurevphysiol_64_0_129_s_31	11826266	( A) The mating factor pheromone binds to a cell surface receptor Ste2 (or Ste3), which  promotes GTP binding to the G protein   subunit (Gpa1).	bind
58298	2	722	5	NULL	NULL	0	NULL	Ste2	GP		is a type of					cell surface receptor	GP				NULL		0	NULL	NULL	NULL	gw70_annurevphysiol_64_0_129_s_31	11826266	( A) The mating factor pheromone binds to a cell surface receptor Ste2 (or Ste3), which  promotes GTP binding to the G protein   subunit (Gpa1).	bind
58299	3	722	5	NULL	NULL	0	NULL	Ste3	GP		is a type of					cell surface receptor	GP				NULL		0	NULL	NULL	NULL	gw70_annurevphysiol_64_0_129_s_31	11826266	( A) The mating factor pheromone binds to a cell surface receptor Ste2 (or Ste3), which  promotes GTP binding to the G protein   subunit (Gpa1).	bind
58300	4	722	5	NULL	NULL	0	NULL	Gpa1	GP		is					G protein subunit	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_64_0_129_s_31	11826266	( A) The mating factor pheromone binds to a cell surface receptor Ste2 (or Ste3), which  promotes GTP binding to the G protein   subunit (Gpa1).	bind
58301	5	722	5	NULL	NULL	0	NULL	pheromone	GP		bind					Ste2	GP				NULL		0	NULL	NULL	NULL	gw70_annurevphysiol_64_0_129_s_31	11826266	( A) The mating factor pheromone binds to a cell surface receptor Ste2 (or Ste3), which  promotes GTP binding to the G protein   subunit (Gpa1).	bind
58302	6	722	5	NULL	NULL	0	NULL	pheromone	GP		bind					Ste3	GP				NULL		0	NULL	NULL	NULL	gw70_annurevphysiol_64_0_129_s_31	11826266	( A) The mating factor pheromone binds to a cell surface receptor Ste2 (or Ste3), which  promotes GTP binding to the G protein   subunit (Gpa1).	bind
58303	7	722	5	NULL	NULL	0	NULL	statement 5	Process		is an alternative to					statement 6	Process				NULL		0	NULL	NULL	NULL	gw70_annurevphysiol_64_0_129_s_31	11826266	( A) The mating factor pheromone binds to a cell surface receptor Ste2 (or Ste3), which  promotes GTP binding to the G protein   subunit (Gpa1).	bind
58304	8	722	5	NULL	NULL	0	NULL	GTP	Chemical		bind					Gpa1	GP				NULL		0	NULL	NULL	NULL	gw70_annurevphysiol_64_0_129_s_31	11826266	( A) The mating factor pheromone binds to a cell surface receptor Ste2 (or Ste3), which  promotes GTP binding to the G protein   subunit (Gpa1).	bind
58305	9	722	5	NULL	NULL	0	NULL	statement 5	Process		promotes					statement 8	Process				NULL		0	NULL	NULL	NULL	gw70_annurevphysiol_64_0_129_s_31	11826266	( A) The mating factor pheromone binds to a cell surface receptor Ste2 (or Ste3), which  promotes GTP binding to the G protein   subunit (Gpa1).	bind
58306	10	722	5	NULL	NULL	0	NULL	statement 6	Process		promotes					statement 8	Process				NULL		0	NULL	NULL	NULL	gw70_annurevphysiol_64_0_129_s_31	11826266	( A) The mating factor pheromone binds to a cell surface receptor Ste2 (or Ste3), which  promotes GTP binding to the G protein   subunit (Gpa1).	bind
1999	1	722	6	NULL	NULL	0	NULL	pheromone	Chemical		bind					Ste2	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_64_0_129_s_31	11826266	( A) The mating factor pheromone binds to a cell surface receptor Ste2 (or Ste3), which  promotes GTP binding to the G protein   subunit (Gpa1).	bind
2000	2	722	6	NULL	NULL	0	NULL	GTP	Chemical		bind					Gpa1	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_64_0_129_s_31	11826266	( A) The mating factor pheromone binds to a cell surface receptor Ste2 (or Ste3), which  promotes GTP binding to the G protein   subunit (Gpa1).	bind
2001	3	722	6	NULL	NULL	0	NULL	Statement 1	Process		promotes					Statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_64_0_129_s_31	11826266	( A) The mating factor pheromone binds to a cell surface receptor Ste2 (or Ste3), which  promotes GTP binding to the G protein   subunit (Gpa1).	bind
51974	4	722	6	NULL	NULL	0	NULL	pheromone	Chemical		bind					Ste3	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_64_0_129_s_31	11826266	( A) The mating factor pheromone binds to a cell surface receptor Ste2 (or Ste3), which  promotes GTP binding to the G protein   subunit (Gpa1).	bind
51975	5	722	6	NULL	NULL	0	NULL	statement 4	Process		promotes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_64_0_129_s_31	11826266	( A) The mating factor pheromone binds to a cell surface receptor Ste2 (or Ste3), which  promotes GTP binding to the G protein   subunit (Gpa1).	bind
51976	6	722	6	NULL	NULL	0	NULL	pheromone	Chemical		is a type of					mating factor	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_64_0_129_s_31	11826266	( A) The mating factor pheromone binds to a cell surface receptor Ste2 (or Ste3), which  promotes GTP binding to the G protein   subunit (Gpa1).	bind
51977	7	722	6	NULL	NULL	0	NULL	Ste2	GP		is a type of					cell surface receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_64_0_129_s_31	11826266	( A) The mating factor pheromone binds to a cell surface receptor Ste2 (or Ste3), which  promotes GTP binding to the G protein   subunit (Gpa1).	bind
51978	8	722	6	NULL	NULL	0	NULL	Ste3	GP		is a type of					cell surface receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_64_0_129_s_31	11826266	( A) The mating factor pheromone binds to a cell surface receptor Ste2 (or Ste3), which  promotes GTP binding to the G protein   subunit (Gpa1).	bind
51979	9	722	6	NULL	NULL	0	NULL	Gpa1	GP		is a type of					G protein subunit	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_64_0_129_s_31	11826266	( A) The mating factor pheromone binds to a cell surface receptor Ste2 (or Ste3), which  promotes GTP binding to the G protein   subunit (Gpa1).	bind
58307	1	724	5	NULL	NULL	0	NULL	Cul1	GP	affinity-purified	bind					GST - CAND1	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_103_31_11515_s_114	16861300	( A) The neddylation of affinity-purified Cul1 bound to GST - CAND1 is stimulated by  Skp2 in the absence of substrate, and the requirement for substrate is restored by  the fraction not adsorbed to GST - CAND1.	bind
58308	2	724	5	NULL	NULL	0	NULL	Skp2 	GP		stimulates					statement 1	GP	neddylation of			NULL		0	NULL	NULL	NULL	gw70_pnas_103_31_11515_s_114	16861300	( A) The neddylation of affinity-purified Cul1 bound to GST - CAND1 is stimulated by  Skp2 in the absence of substrate, and the requirement for substrate is restored by  the fraction not adsorbed to GST - CAND1.	bind
2002	1	724	6	NULL	NULL	0	NULL	Cul1	GP	purified	bind					GST-CAND1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_31_11515_s_114	16861300	( A) The neddylation of affinity-purified Cul1 bound to GST - CAND1 is stimulated by  Skp2 in the absence of substrate, and the requirement for substrate is restored by  the fraction not adsorbed to GST - CAND1.	bind
2003	2	724	6	NULL	NULL	0	NULL	Skp2	GP		stimulates					Statement 1	Process	neddylation			NULL	in the absence of substrate	NULL	NULL	NULL	NULL	gw70_pnas_103_31_11515_s_114	16861300	( A) The neddylation of affinity-purified Cul1 bound to GST - CAND1 is stimulated by  Skp2 in the absence of substrate, and the requirement for substrate is restored by  the fraction not adsorbed to GST - CAND1.	bind
58309	1	725	5	NULL	NULL	0	NULL	NF-kappaB complex	GP		bind					Bcl-x	GP			putative NF-kappaB-binding sites in promoter	NULL		0	NULL	NULL	NULL	gw60_pnas_96_16_9136_s_133	10430908	( A) The NF-kappaB complex binding to the putative NF-kappaB-binding sites within the Bcl-x promoter consists predominantly of p50, p65, and c-Rel.	bind
58310	2	725	5	NULL	NULL	0	NULL	NF-kappaB complex	GP		consists of					p50	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_96_16_9136_s_133	10430908	( A) The NF-kappaB complex binding to the putative NF-kappaB-binding sites within the Bcl-x promoter consists predominantly of p50, p65, and c-Rel.	bind
58311	3	725	5	NULL	NULL	0	NULL	NF-kappaB complex	GP		consists of					p65	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_96_16_9136_s_133	10430908	( A) The NF-kappaB complex binding to the putative NF-kappaB-binding sites within the Bcl-x promoter consists predominantly of p50, p65, and c-Rel.	bind
58312	4	725	5	NULL	NULL	0	NULL	NF-kappaB complex	GP		consists of					c-Rel	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_96_16_9136_s_133	10430908	( A) The NF-kappaB complex binding to the putative NF-kappaB-binding sites within the Bcl-x promoter consists predominantly of p50, p65, and c-Rel.	bind
2004	1	725	6	NULL	NULL	0	NULL	p50	GP		bind					BCL-x	GP			NF-kappaB-binding sites of promoter	NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_16_9136_s_133	10430908	( A) The NF-kappaB complex binding to the putative NF-kappaB-binding sites within the Bcl-x promoter consists predominantly of p50, p65, and c-Rel.	bind
2005	2	725	6	NULL	NULL	0	NULL	p65	GP		bind					BCL-x	GP			NF-kappaB-binding sites of promoter	NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_16_9136_s_133	10430908	( A) The NF-kappaB complex binding to the putative NF-kappaB-binding sites within the Bcl-x promoter consists predominantly of p50, p65, and c-Rel.	bind
2006	3	725	6	NULL	NULL	0	NULL	c-rel	GP		bind					BCL-x	GP			NF-kappaB-binding sites of promoter	NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_16_9136_s_133	10430908	( A) The NF-kappaB complex binding to the putative NF-kappaB-binding sites within the Bcl-x promoter consists predominantly of p50, p65, and c-Rel.	bind
58313	1	726	5	NULL	NULL	0	NULL	Hsp72	GP		bind					JNK1	GP				NULL	in vitro	0	NULL	NULL	NULL	gw60_embo_20_3_446_s_129	11157751	( A) The peptide binding domain is essential for Hsp72 binding to JNK1  in vitro.	bind
2007	1	726	6	NULL	NULL	0	NULL	Hsp72	GP		bind					JNK1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_20_3_446_s_129	11157751	( A) The peptide binding domain is essential for Hsp72 binding to JNK1  in vitro.	bind
2008	2	726	6	NULL	NULL	0	NULL		GP		is essential for			peptide binding domain		Statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_20_3_446_s_129	11157751	( A) The peptide binding domain is essential for Hsp72 binding to JNK1  in vitro.	bind
58314	1	728	5	NULL	NULL	0	NULL	PIASy	GP		bind			SAP domain		MAR DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_genesdev_15_23_3088_s_238	11731474	( A) The PIASy SAP domain binds to MAR DNA.	bind
2009	1	728	6	NULL	NULL	0	NULL	PIASy	GP		bind			SAP domain		MAR DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_23_3088_s_238	11731474	( A) The PIASy SAP domain binds to MAR DNA.	bind
58315	1	729	5	NULL	NULL	0	NULL	Pit-1 homodimer	GP		bind			POU domain					prolactin Prl-1P site		NULL		0	NULL	NULL	NULL	gw60_science_290_5494_1127_s_52	11073444	( A) The Pit-1 POU domain homodimer is  bound to the prolactin Prl-1P (left) and the growth hormone GH-1  (right) sites.	bind
58316	2	729	5	NULL	NULL	0	NULL	Pit-1 homodimer	GP		bind			POU domain					GH-1 site		NULL		0	NULL	NULL	NULL	gw60_science_290_5494_1127_s_52	11073444	( A) The Pit-1 POU domain homodimer is  bound to the prolactin Prl-1P (left) and the growth hormone GH-1  (right) sites.	bind
58317	3	729	5	NULL	NULL	0	NULL	GH-1	GP		is a type of					growth hormone	GP				NULL		0	NULL	NULL	NULL	gw60_science_290_5494_1127_s_52	11073444	( A) The Pit-1 POU domain homodimer is  bound to the prolactin Prl-1P (left) and the growth hormone GH-1  (right) sites.	bind
2010	1	729	6	NULL	NULL	0	NULL	Pit-1 homodimer	GP		bind			POU domain		Prl-1P	GP			sites	NULL		NULL	NULL	NULL	NULL	gw60_science_290_5494_1127_s_52	11073444	( A) The Pit-1 POU domain homodimer is  bound to the prolactin Prl-1P (left) and the growth hormone GH-1  (right) sites.	bind
2011	2	729	6	NULL	NULL	0	NULL	Pit-1 homodimer	GP		bind			POU domain		GH-1	GP			sites	NULL		NULL	NULL	NULL	NULL	gw60_science_290_5494_1127_s_52	11073444	( A) The Pit-1 POU domain homodimer is  bound to the prolactin Prl-1P (left) and the growth hormone GH-1  (right) sites.	bind
51980	3	729	6	NULL	NULL	0	NULL	Prl-1P	GP		is					prolactin	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_290_5494_1127_s_52	11073444	( A) The Pit-1 POU domain homodimer is  bound to the prolactin Prl-1P (left) and the growth hormone GH-1  (right) sites.	bind
51981	4	729	6	NULL	NULL	0	NULL	GH-1	GP		is					growth hormone	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_290_5494_1127_s_52	11073444	( A) The Pit-1 POU domain homodimer is  bound to the prolactin Prl-1P (left) and the growth hormone GH-1  (right) sites.	bind
58318	1	731	5	NULL	NULL	0	NULL	RdRp	GP		bind					RdRp	NucleicAcid			promoter	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_11_2824_s_171	12771209	( A) The RdRp can bind to both the vRNA and cRNA promoters.	bind
58319	2	731	5	NULL	NULL	0	NULL	RdRp	GP		bind					cRNA	NucleicAcid			promoter	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_11_2824_s_171	12771209	( A) The RdRp can bind to both the vRNA and cRNA promoters.	bind
2012	1	731	6	NULL	NULL	0	NULL	RdRp	GP		bind					vRNA	GP			Promoter	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_11_2824_s_171	12771209	( A) The RdRp can bind to both the vRNA and cRNA promoters.	bind
2013	2	731	6	NULL	NULL	0	NULL	RdRp	GP		bind					cRNA	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_11_2824_s_171	12771209	( A) The RdRp can bind to both the vRNA and cRNA promoters.	bind
58320	1	732	5	NULL	NULL	0	NULL	RepE monomer	GP		bind					ori2 iterons	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_embo_18_13_3856_s_19	10393200	( A) The RepE monomer binds to the four  ori2 iterons [direct repeats (DR)].	bind
2014	1	732	6	NULL	NULL	0	NULL	RepE	GP	monomer	bind					four ori2 iterons				DR	NULL		NULL	NULL	NULL	NULL	gw60_embo_18_13_3856_s_19	10393200	( A) The RepE monomer binds to the four  ori2 iterons [direct repeats (DR)].	bind
51982	2	732	6	10	NULL	0	NULL	DR	NULL		is	NULL				direct repeat	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_18_13_3856_s_19	10393200	( A) The RepE monomer binds to the four  ori2 iterons [direct repeats (DR)].	bind
58321	1	734	5	NULL	NULL	0	NULL	Pax6deltaHD	GP	wild-type	bind					GST-HD	GP				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_8_2661_s_205	15886395	( A) The single mutants of Pax6deltaHD, E112A, E120A and E128A bind to GST-HD with the same affinity as the wild type.	bind
58322	2	734	5	NULL	NULL	0	NULL	Pax6deltaHD	GP	mutant	bind			E112A		GST-HD	GP				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_8_2661_s_205	15886395	( A) The single mutants of Pax6deltaHD, E112A, E120A and E128A bind to GST-HD with the same affinity as the wild type.	bind
58323	3	734	5	NULL	NULL	0	NULL	Pax6deltaHD	GP	mutant	bind			E120A		GST-HD	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_8_2661_s_205	15886395	( A) The single mutants of Pax6deltaHD, E112A, E120A and E128A bind to GST-HD with the same affinity as the wild type.	bind
58324	4	734	5	NULL	NULL	0	NULL	Pax6deltaHD	GP	mutant	bind			E128A		GST-HD	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_8_2661_s_205	15886395	( A) The single mutants of Pax6deltaHD, E112A, E120A and E128A bind to GST-HD with the same affinity as the wild type.	bind
58325	5	734	5	NULL	NULL	0	NULL	statement 2	Process		same affinity as					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_8_2661_s_205	15886395	( A) The single mutants of Pax6deltaHD, E112A, E120A and E128A bind to GST-HD with the same affinity as the wild type.	bind
58326	6	734	5	NULL	NULL	0	NULL	statement 3	Process		same affinity as					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_8_2661_s_205	15886395	( A) The single mutants of Pax6deltaHD, E112A, E120A and E128A bind to GST-HD with the same affinity as the wild type.	bind
58327	7	734	5	NULL	NULL	0	NULL	statement 4	Process		same affinity as					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_8_2661_s_205	15886395	( A) The single mutants of Pax6deltaHD, E112A, E120A and E128A bind to GST-HD with the same affinity as the wild type.	bind
2015	1	734	6	NULL	NULL	0	NULL	Pax6delta	GP		bind			mutant HD		GST-HD	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_8_2661_s_205	15886395	( A) The single mutants of Pax6deltaHD, E112A, E120A and E128A bind to GST-HD with the same affinity as the wild type.	bind
2016	2	734	6	NULL	NULL	0	NULL	Pax6delta	GP		bind			mutant E112A		GST-HD	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_8_2661_s_205	15886395	( A) The single mutants of Pax6deltaHD, E112A, E120A and E128A bind to GST-HD with the same affinity as the wild type.	bind
2017	3	734	6	NULL	NULL	0	NULL	Pax6delta	GP		bind			mutant E120A		GST-HD	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_8_2661_s_205	15886395	( A) The single mutants of Pax6deltaHD, E112A, E120A and E128A bind to GST-HD with the same affinity as the wild type.	bind
2018	4	734	6	NULL	NULL	0	NULL	Pax6delta	GP		bind			mutant E128A		GST-HD	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_8_2661_s_205	15886395	( A) The single mutants of Pax6deltaHD, E112A, E120A and E128A bind to GST-HD with the same affinity as the wild type.	bind
54098	5	734	6	NULL	NULL	0	NULL	Pax6delta	GP	wild type	bind					GST-HD	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_8_2661_s_205	15886395	( A) The single mutants of Pax6deltaHD, E112A, E120A and E128A bind to GST-HD with the same affinity as the wild type.	bind
58328	1	735	5	NULL	NULL	0	NULL	REST/NRSF	GP		is a type of					transcriptional repressor	GP				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_17_3403_s_46	10954611	( A) The transcriptional repressor REST/NRSF contains a DNA-binding domain (Zn-DBD), consisting of eight zinc finger motifs, that bind to the consensus RE1 (or NRSE) sequence.	bind
58329	2	735	5	NULL	NULL	0	NULL	REST/NRSF	GP		bind			Zn-DBD		RE1 sequence	NucleicAcid	consensus			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_17_3403_s_46	10954611	( A) The transcriptional repressor REST/NRSF contains a DNA-binding domain (Zn-DBD), consisting of eight zinc finger motifs, that bind to the consensus RE1 (or NRSE) sequence.	bind
58330	3	735	5	NULL	NULL	0	NULL	REST/NRSF	GP		bind			Zn-DBD		NRSE sequence	NucleicAcid	consensus			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_17_3403_s_46	10954611	( A) The transcriptional repressor REST/NRSF contains a DNA-binding domain (Zn-DBD), consisting of eight zinc finger motifs, that bind to the consensus RE1 (or NRSE) sequence.	bind
58331	4	735	5	NULL	NULL	0	NULL	Zn-DBD	AminoAcid		is					DNA-binding domain	AminoAcid				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_17_3403_s_46	10954611	( A) The transcriptional repressor REST/NRSF contains a DNA-binding domain (Zn-DBD), consisting of eight zinc finger motifs, that bind to the consensus RE1 (or NRSE) sequence.	bind
2019	1	735	6	NULL	NULL	0	NULL	REST/NRSF	GP		bind			Zn-DBD			NucleicAcid			consensus RE1 sequence	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_17_3403_s_46	10954611	( A) The transcriptional repressor REST/NRSF contains a DNA-binding domain (Zn-DBD), consisting of eight zinc finger motifs, that bind to the consensus RE1 (or NRSE) sequence.	bind
2020	2	735	6	NULL	NULL	0	NULL		GP		consist of 			Zn-DBD		eight zinc finger motifs	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_17_3403_s_46	10954611	( A) The transcriptional repressor REST/NRSF contains a DNA-binding domain (Zn-DBD), consisting of eight zinc finger motifs, that bind to the consensus RE1 (or NRSE) sequence.	bind
51983	3	735	6	NULL	NULL	0	NULL	REST/NRSF	GP		bind			Zn-DBD			NucleicAcid			consensus NRSE sequence	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_17_3403_s_46	10954611	( A) The transcriptional repressor REST/NRSF contains a DNA-binding domain (Zn-DBD), consisting of eight zinc finger motifs, that bind to the consensus RE1 (or NRSE) sequence.	bind
51984	4	735	6	NULL	NULL	0	NULL	REST/NRSF	GP		is a type of					transcriptional repressor	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_17_3403_s_46	10954611	( A) The transcriptional repressor REST/NRSF contains a DNA-binding domain (Zn-DBD), consisting of eight zinc finger motifs, that bind to the consensus RE1 (or NRSE) sequence.	bind
51985	5	735	6	NULL	NULL	0	NULL	Zn-DBD	GP		is					DNA-binding domain	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_17_3403_s_46	10954611	( A) The transcriptional repressor REST/NRSF contains a DNA-binding domain (Zn-DBD), consisting of eight zinc finger motifs, that bind to the consensus RE1 (or NRSE) sequence.	bind
58332	1	736	5	NULL	NULL	0	NULL	stathmin/OP18	GP	truncated	bind					alpha-tubulin	GP				NULL		0	NULL	NULL	NULL	gw60_embo_19_2_213_s_191	10637225	( A) The truncated forms of stathmin/OP18 bind only to one alpha-tubulin of the heterodimer.	bind
2021	1	736	6	NULL	NULL	0	NULL	stathmin/OP18	GP	truncated	bind					alpha-tubulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_2_213_s_191	10637225	( A) The truncated forms of stathmin/OP18 bind only to one alpha-tubulin of the heterodimer.	bind
58333	1	739	5	NULL	NULL	0	NULL	U1C	GP		bind					U1 RNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_pnas_101_41_14841_s_179	15465910	( A) There is little U1C binding to U1 RNA at low temperature, because of a favored RNA  - RNA interaction, depicted as an intramolecular base-pairing interaction between  a putative ps5'' and the 5'ss.	bind
2022	1	739	6	NULL	NULL	0	NULL	U1C	GP		bind		low			U1RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_41_14841_s_179	15465910	( A) There is little U1C binding to U1 RNA at low temperature, because of a favored RNA  - RNA interaction, depicted as an intramolecular base-pairing interaction between  a putative ps5'' and the 5'ss.	bind
2023	2	739	6	NULL	NULL	0	NULL	ps5	NucleicAcid	putative	base pairs with					5'ss	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_41_14841_s_179	15465910	( A) There is little U1C binding to U1 RNA at low temperature, because of a favored RNA  - RNA interaction, depicted as an intramolecular base-pairing interaction between  a putative ps5'' and the 5'ss.	bind
51986	3	739	6	NULL	NULL	0	NULL	RNA	NucleicAcid		interacts with					RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_41_14841_s_179	15465910	( A) There is little U1C binding to U1 RNA at low temperature, because of a favored RNA  - RNA interaction, depicted as an intramolecular base-pairing interaction between  a putative ps5'' and the 5'ss.	bind
51987	4	739	6	NULL	NULL	0	NULL	statement 1	Process		because of					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_41_14841_s_179	15465910	( A) There is little U1C binding to U1 RNA at low temperature, because of a favored RNA  - RNA interaction, depicted as an intramolecular base-pairing interaction between  a putative ps5'' and the 5'ss.	bind
51988	5	739	6	NULL	NULL	0	NULL	statement 3	Process		depicted as					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_41_14841_s_179	15465910	( A) There is little U1C binding to U1 RNA at low temperature, because of a favored RNA  - RNA interaction, depicted as an intramolecular base-pairing interaction between  a putative ps5'' and the 5'ss.	bind
58334	1	740	5	NULL	NULL	0	NULL	Bak	GP		bind		tightly	BH3		Mcl-1	GP				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1294_s_101	15901672	( A) Tight binding of Bak BH3 to Mcl-1 and Bcl-xL.	bind
58335	2	740	5	NULL	NULL	0	NULL	Bak	GP		bind		tightly	BH3		Bcl-xL	GP				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1294_s_101	15901672	( A) Tight binding of Bak BH3 to Mcl-1 and Bcl-xL.	bind
2024	1	740	6	NULL	NULL	0	NULL	Bak	GP		bind		tightly	BH3		Mcl-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_11_1294_s_101	15901672	( A) Tight binding of Bak BH3 to Mcl-1 and Bcl-xL.	bind
2025	2	740	6	NULL	NULL	0	NULL	Bak	GP		bind		tightly	BH3		Bcl-xL	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_11_1294_s_101	15901672	( A) Tight binding of Bak BH3 to Mcl-1 and Bcl-xL.	bind
58336	1	742	5	NULL	NULL	0	NULL	TIP47	GP		bind					CI-MPR	GP				NULL		0	NULL	NULL	NULL	gw60_science_292_5520_1373_s_62	11359012	( A) TIP47 binds both CI-MPR and Rab9 in a ternary complex.	bind
58337	2	742	5	NULL	NULL	0	NULL	TIP47	GP		bind					Rab9	GP				NULL		0	NULL	NULL	NULL	gw60_science_292_5520_1373_s_62	11359012	( A) TIP47 binds both CI-MPR and Rab9 in a ternary complex.	bind
2026	1	742	6	NULL	NULL	0	NULL	TIP47	GP		bind					CI-MPR	GP				NULL	ternary complex	NULL	NULL	NULL	NULL	gw60_science_292_5520_1373_s_62	11359012	( A) TIP47 binds both CI-MPR and Rab9 in a ternary complex.	bind
2027	2	742	6	NULL	NULL	0	NULL	TIP47	GP		bind					Rab9	GP				NULL	ternary complex	NULL	NULL	NULL	NULL	gw60_science_292_5520_1373_s_62	11359012	( A) TIP47 binds both CI-MPR and Rab9 in a ternary complex.	bind
58338	1	743	5	NULL	NULL	0	NULL	TMEFF1	GP		bind					Cripto	GP				NULL	CHO cells	0	NULL	NULL	NULL	gw70_genesdev_17_21_2624_s_129	14563676	( A) TMEFF1 binds to Cripto in CHO cells.	bind
2028	1	743	6	NULL	NULL	0	NULL	TMEFF1	GP		bind					Cripto	GP				NULL	CHO cells	NULL	NULL	NULL	NULL	gw70_genesdev_17_21_2624_s_129	14563676	( A) TMEFF1 binds to Cripto in CHO cells.	bind
58339	1	744	5	NULL	NULL	0	NULL	IKK	GP		triggers					IkappaB	GP	phosphorylation of			NULL		0	NULL	NULL	NULL	gw70_embo_24_3_510_s_165	15660126	( A) TNFalpha signals to IKK to trigger IkappaB phosphorylation and degradation, thereby eliciting NF-kappaB nuclear translocation, DNA binding and transcriptional repression of EAAT2.	bind
58340	2	744	5	NULL	NULL	0	NULL	statement 1	Process		leads to					IkappaB	GP	degradation of			NULL		0	NULL	NULL	NULL	gw70_embo_24_3_510_s_165	15660126	( A) TNFalpha signals to IKK to trigger IkappaB phosphorylation and degradation, thereby eliciting NF-kappaB nuclear translocation, DNA binding and transcriptional repression of EAAT2.	bind
58341	3	744	5	NULL	NULL	0	NULL	TNFalpha	GP		signals					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_embo_24_3_510_s_165	15660126	( A) TNFalpha signals to IKK to trigger IkappaB phosphorylation and degradation, thereby eliciting NF-kappaB nuclear translocation, DNA binding and transcriptional repression of EAAT2.	bind
58342	4	744	5	NULL	NULL	0	NULL	NF-kappaB	GP		is translocated to					nucleus	CellComponent				NULL		0	NULL	NULL	NULL	gw70_embo_24_3_510_s_165	15660126	( A) TNFalpha signals to IKK to trigger IkappaB phosphorylation and degradation, thereby eliciting NF-kappaB nuclear translocation, DNA binding and transcriptional repression of EAAT2.	bind
58343	5	744	5	NULL	NULL	0	NULL	statement 2	Process		elicits					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_embo_24_3_510_s_165	15660126	( A) TNFalpha signals to IKK to trigger IkappaB phosphorylation and degradation, thereby eliciting NF-kappaB nuclear translocation, DNA binding and transcriptional repression of EAAT2.	bind
58344	6	744	5	NULL	NULL	0	NULL	NF-kappaB	GP		bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_embo_24_3_510_s_165	15660126	( A) TNFalpha signals to IKK to trigger IkappaB phosphorylation and degradation, thereby eliciting NF-kappaB nuclear translocation, DNA binding and transcriptional repression of EAAT2.	bind
58345	7	744	5	NULL	NULL	0	NULL	statement 2	Process		elicits					statement 6	Process				NULL		0	NULL	NULL	NULL	gw70_embo_24_3_510_s_165	15660126	( A) TNFalpha signals to IKK to trigger IkappaB phosphorylation and degradation, thereby eliciting NF-kappaB nuclear translocation, DNA binding and transcriptional repression of EAAT2.	bind
58346	8	744	5	NULL	NULL	0	NULL	statement 2	Process		repress					EAAT2	GP	transcription of			NULL		0	NULL	NULL	NULL	gw70_embo_24_3_510_s_165	15660126	( A) TNFalpha signals to IKK to trigger IkappaB phosphorylation and degradation, thereby eliciting NF-kappaB nuclear translocation, DNA binding and transcriptional repression of EAAT2.	bind
2167	2	744	6	NULL	NULL	0	NULL	statement 1	Process		trigger					IkappaB	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw70_embo_24_3_510_s_165	15660126	( A) TNFalpha signals to IKK to trigger IkappaB phosphorylation and degradation, thereby eliciting NF-kappaB nuclear translocation, DNA binding and transcriptional repression of EAAT2.	bind
2168	3	744	6	NULL	NULL	0	NULL	statement 1	Process		trigger					IkappaB	GP	degradation of			NULL		NULL	NULL	NULL	NULL	gw70_embo_24_3_510_s_165	15660126	( A) TNFalpha signals to IKK to trigger IkappaB phosphorylation and degradation, thereby eliciting NF-kappaB nuclear translocation, DNA binding and transcriptional repression of EAAT2.	bind
2169	1	744	6	NULL	NULL	0	NULL	TNFalpha	GP		signals					 IKK	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_3_510_s_165	15660126	( A) TNFalpha signals to IKK to trigger IkappaB phosphorylation and degradation, thereby eliciting NF-kappaB nuclear translocation, DNA binding and transcriptional repression of EAAT2.	bind
2194	4	744	6	NULL	NULL	0	NULL	NF-kappaB	GP		is translocated to					nucleus	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_3_510_s_165	15660126	( A) TNFalpha signals to IKK to trigger IkappaB phosphorylation and degradation, thereby eliciting NF-kappaB nuclear translocation, DNA binding and transcriptional repression of EAAT2.	bind
2195	5	744	6	NULL	NULL	0	NULL	NF-kappaB	GP		bind					EAAT2	GP			DNA	NULL		NULL	NULL	NULL	NULL	gw70_embo_24_3_510_s_165	15660126	( A) TNFalpha signals to IKK to trigger IkappaB phosphorylation and degradation, thereby eliciting NF-kappaB nuclear translocation, DNA binding and transcriptional repression of EAAT2.	bind
2196	6	744	6	NULL	NULL	0	NULL	NF-kappaB	GP		represses					EAAT2	GP	transcription of 			NULL		NULL	NULL	NULL	NULL	gw70_embo_24_3_510_s_165	15660126	( A) TNFalpha signals to IKK to trigger IkappaB phosphorylation and degradation, thereby eliciting NF-kappaB nuclear translocation, DNA binding and transcriptional repression of EAAT2.	bind
2197	7	744	6	NULL	NULL	0	NULL	statement 2	Process		occur along with					Statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_3_510_s_165	15660126	( A) TNFalpha signals to IKK to trigger IkappaB phosphorylation and degradation, thereby eliciting NF-kappaB nuclear translocation, DNA binding and transcriptional repression of EAAT2.	bind
2198	8	744	6	NULL	NULL	0	NULL	statement 7	Process		elicits					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_3_510_s_165	15660126	( A) TNFalpha signals to IKK to trigger IkappaB phosphorylation and degradation, thereby eliciting NF-kappaB nuclear translocation, DNA binding and transcriptional repression of EAAT2.	bind
2199	9	744	6	NULL	NULL	0	NULL	statement 7	Process		elicits					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_3_510_s_165	15660126	( A) TNFalpha signals to IKK to trigger IkappaB phosphorylation and degradation, thereby eliciting NF-kappaB nuclear translocation, DNA binding and transcriptional repression of EAAT2.	bind
51989	10	744	6	NULL	NULL	0	NULL	statement 7	Process		elicits					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_3_510_s_165	15660126	( A) TNFalpha signals to IKK to trigger IkappaB phosphorylation and degradation, thereby eliciting NF-kappaB nuclear translocation, DNA binding and transcriptional repression of EAAT2.	bind
58347	1	749	5	NULL	NULL	0	NULL	tPA	GP		bind					PDGF-CC	GP	latent	CUB domain;;growth factor domain		NULL		0	NULL	NULL	NULL	gw70_embo_23_19_3793_s_188	15372073	( A) tPA binds to both the CUB domain and the growth factor domain of latent PDGF-CC.	bind
2029	1	749	6	NULL	NULL	0	NULL	tPA	GP		bind					PDGF-CC	GP	latent	CUB domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_19_3793_s_188	15372073	( A) tPA binds to both the CUB domain and the growth factor domain of latent PDGF-CC.	bind
2030	2	749	6	NULL	NULL	0	NULL	tPA	GP		bind					PDGF-CC	GP	latent	growth factor domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_19_3793_s_188	15372073	( A) tPA binds to both the CUB domain and the growth factor domain of latent PDGF-CC.	bind
58348	1	750	5	NULL	NULL	0	NULL	TPP1	GP		bind		directly			TIN2	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_103_32_11874_s_107	16880378	( a) TPP1 directly binds TIN2 but not TRF2.	bind
58349	2	750	5	NULL	NULL	0	NULL	TPP1	GP		does not bind					TRF2	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_32_11874_s_107	16880378	( a) TPP1 directly binds TIN2 but not TRF2.	bind
2031	1	750	6	NULL	NULL	0	NULL	TPP1	GP		bind		directly			TIN2	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_32_11874_s_107	16880378	( a) TPP1 directly binds TIN2 but not TRF2.	bind
2032	2	750	6	NULL	NULL	0	NULL	TPP1	GP		does not bind		directly			TRF2	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_32_11874_s_107	16880378	( a) TPP1 directly binds TIN2 but not TRF2.	bind
2035	1	751	6	NULL	NULL	0	NULL	TRAF6	GP		bind					Cyt-N	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_4_1234_s_93	9990007	( A) TRAF6 binding with cyt-N was abolished by the QE234-5AA mutation.	bind
2036	2	751	6	NULL	NULL	0	NULL	TRAF6	GP		abolishes			QE234-5AA mutant		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_4_1234_s_93	9990007	( A) TRAF6 binding with cyt-N was abolished by the QE234-5AA mutation.	bind
58351	1	753	5	NULL	NULL	0	NULL	Rab	GP		bind					GDI/REP	GP				NULL		0	NULL	NULL	NULL	gw70_embo_25_1_13_s_181	16395334	( A) Two-step binding of Rab to GDI/REP.	bind
2034	1	753	6	NULL	NULL	0	NULL	Rab	GP		bind					GDI/REP	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_1_13_s_181	16395334	( A) Two-step binding of Rab to GDI/REP.	bind
58352	1	754	5	NULL	NULL	0	NULL	U1 snRNP	GP		bind					dsx pre-mRNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_pnas_96_11_6125_s_111	10339552	( A) U1 snRNP binds to the  dsx pre-mRNA independently of the ESE, whereas the ESE and U1 snRNP are required for the assembly of U2, U4/U6, and U5 snRNPs on the  dsx pre-mRNA.	bind
58353	2	754	5	NULL	NULL	0	NULL	statement 1	Process		is independent of					ESE	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_pnas_96_11_6125_s_111	10339552	( A) U1 snRNP binds to the  dsx pre-mRNA independently of the ESE, whereas the ESE and U1 snRNP are required for the assembly of U2, U4/U6, and U5 snRNPs on the  dsx pre-mRNA.	bind
58354	3	754	5	NULL	NULL	0	NULL	U2	GP		assemble on					dsx pre-mRNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_pnas_96_11_6125_s_111	10339552	( A) U1 snRNP binds to the  dsx pre-mRNA independently of the ESE, whereas the ESE and U1 snRNP are required for the assembly of U2, U4/U6, and U5 snRNPs on the  dsx pre-mRNA.	bind
58355	4	754	5	NULL	NULL	0	NULL	U4/U6	GP		assemble on					dsx pre-mRNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_pnas_96_11_6125_s_111	10339552	( A) U1 snRNP binds to the  dsx pre-mRNA independently of the ESE, whereas the ESE and U1 snRNP are required for the assembly of U2, U4/U6, and U5 snRNPs on the  dsx pre-mRNA.	bind
58356	5	754	5	NULL	NULL	0	NULL	U5 snRNPs	GP		assemble on					dsx pre-mRNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_pnas_96_11_6125_s_111	10339552	( A) U1 snRNP binds to the  dsx pre-mRNA independently of the ESE, whereas the ESE and U1 snRNP are required for the assembly of U2, U4/U6, and U5 snRNPs on the  dsx pre-mRNA.	bind
58357	6	754	5	NULL	NULL	0	NULL	ESE	NucleicAcid		is required for					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_96_11_6125_s_111	10339552	( A) U1 snRNP binds to the  dsx pre-mRNA independently of the ESE, whereas the ESE and U1 snRNP are required for the assembly of U2, U4/U6, and U5 snRNPs on the  dsx pre-mRNA.	bind
58358	7	754	5	NULL	NULL	0	NULL	ESE	NucleicAcid		is required for					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_96_11_6125_s_111	10339552	( A) U1 snRNP binds to the  dsx pre-mRNA independently of the ESE, whereas the ESE and U1 snRNP are required for the assembly of U2, U4/U6, and U5 snRNPs on the  dsx pre-mRNA.	bind
58359	8	754	5	NULL	NULL	0	NULL	ESE	NucleicAcid		is required for					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_96_11_6125_s_111	10339552	( A) U1 snRNP binds to the  dsx pre-mRNA independently of the ESE, whereas the ESE and U1 snRNP are required for the assembly of U2, U4/U6, and U5 snRNPs on the  dsx pre-mRNA.	bind
58360	9	754	5	NULL	NULL	0	NULL	U1 snRNP	GP		is required for					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_96_11_6125_s_111	10339552	( A) U1 snRNP binds to the  dsx pre-mRNA independently of the ESE, whereas the ESE and U1 snRNP are required for the assembly of U2, U4/U6, and U5 snRNPs on the  dsx pre-mRNA.	bind
58361	10	754	5	NULL	NULL	0	NULL	U1 snRNP	GP		is required for					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_96_11_6125_s_111	10339552	( A) U1 snRNP binds to the  dsx pre-mRNA independently of the ESE, whereas the ESE and U1 snRNP are required for the assembly of U2, U4/U6, and U5 snRNPs on the  dsx pre-mRNA.	bind
58362	11	754	5	NULL	NULL	0	NULL	U1 snRNP	GP		is required for					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_96_11_6125_s_111	10339552	( A) U1 snRNP binds to the  dsx pre-mRNA independently of the ESE, whereas the ESE and U1 snRNP are required for the assembly of U2, U4/U6, and U5 snRNPs on the  dsx pre-mRNA.	bind
2173	1	754	6	NULL	NULL	0	NULL	U1 snRNP	GP		bind					dsx pre-mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_11_6125_s_111	10339552	( A) U1 snRNP binds to the  dsx pre-mRNA independently of the ESE, whereas the ESE and U1 snRNP are required for the assembly of U2, U4/U6, and U5 snRNPs on the  dsx pre-mRNA.	bind
2174	2	754	6	NULL	NULL	0	NULL	statement 1	Process		independent of					ESE	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_11_6125_s_111	10339552	( A) U1 snRNP binds to the  dsx pre-mRNA independently of the ESE, whereas the ESE and U1 snRNP are required for the assembly of U2, U4/U6, and U5 snRNPs on the  dsx pre-mRNA.	bind
2175	3	754	6	NULL	NULL	0	NULL	U2 snRNP	GP		assembles on					dsx pre-mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_11_6125_s_111	10339552	( A) U1 snRNP binds to the  dsx pre-mRNA independently of the ESE, whereas the ESE and U1 snRNP are required for the assembly of U2, U4/U6, and U5 snRNPs on the  dsx pre-mRNA.	bind
2178	4	754	6	NULL	NULL	0	NULL	U4/U6 snRNP	GP		assembles on					dsx pre-mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_11_6125_s_111	10339552	( A) U1 snRNP binds to the  dsx pre-mRNA independently of the ESE, whereas the ESE and U1 snRNP are required for the assembly of U2, U4/U6, and U5 snRNPs on the  dsx pre-mRNA.	bind
51990	5	754	6	NULL	NULL	0	NULL	U5 snRNP	GP		assembles on					dsx pre-mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_11_6125_s_111	10339552	( A) U1 snRNP binds to the  dsx pre-mRNA independently of the ESE, whereas the ESE and U1 snRNP are required for the assembly of U2, U4/U6, and U5 snRNPs on the  dsx pre-mRNA.	bind
51991	6	754	6	NULL	NULL	0	NULL	ESE	GP		is required for 					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_11_6125_s_111	10339552	( A) U1 snRNP binds to the  dsx pre-mRNA independently of the ESE, whereas the ESE and U1 snRNP are required for the assembly of U2, U4/U6, and U5 snRNPs on the  dsx pre-mRNA.	bind
51992	7	754	6	NULL	NULL	0	NULL	ESE	GP		is required for					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_11_6125_s_111	10339552	( A) U1 snRNP binds to the  dsx pre-mRNA independently of the ESE, whereas the ESE and U1 snRNP are required for the assembly of U2, U4/U6, and U5 snRNPs on the  dsx pre-mRNA.	bind
51993	8	754	6	NULL	NULL	0	NULL	ESE	GP		is required for					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_11_6125_s_111	10339552	( A) U1 snRNP binds to the  dsx pre-mRNA independently of the ESE, whereas the ESE and U1 snRNP are required for the assembly of U2, U4/U6, and U5 snRNPs on the  dsx pre-mRNA.	bind
51994	9	754	6	NULL	NULL	0	NULL	U1 snRNP	GP		is required for					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_11_6125_s_111	10339552	( A) U1 snRNP binds to the  dsx pre-mRNA independently of the ESE, whereas the ESE and U1 snRNP are required for the assembly of U2, U4/U6, and U5 snRNPs on the  dsx pre-mRNA.	bind
51995	10	754	6	NULL	NULL	0	NULL	U1 snRNP	GP		is required for					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_11_6125_s_111	10339552	( A) U1 snRNP binds to the  dsx pre-mRNA independently of the ESE, whereas the ESE and U1 snRNP are required for the assembly of U2, U4/U6, and U5 snRNPs on the  dsx pre-mRNA.	bind
51996	11	754	6	NULL	NULL	0	NULL	U1 snRNP	GP		is required for					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_11_6125_s_111	10339552	( A) U1 snRNP binds to the  dsx pre-mRNA independently of the ESE, whereas the ESE and U1 snRNP are required for the assembly of U2, U4/U6, and U5 snRNPs on the  dsx pre-mRNA.	bind
58363	1	755	5	NULL	NULL	0	NULL	GST - Grb2	GP	WT;;unphosphorylated	bind			C-SH3		Sos peptide	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_23_6793_s_121	11726515	( A) Unphosphorylated GST - Grb2-C-SH3 WT or mutant fusion proteins bind Sos peptide beads.	bind
58364	2	755	5	NULL	NULL	0	NULL	GST - Grb2	GP	mutant;;unphosphorylated	bind			C-SH3		Sos peptide	AminoAcid				NULL		0	NULL	NULL	NULL	gw60_embo_20_23_6793_s_121	11726515	( A) Unphosphorylated GST - Grb2-C-SH3 WT or mutant fusion proteins bind Sos peptide beads.	bind
58365	1	756	5	NULL	NULL	0	NULL	Kss1	GP	unphosphorylated	bind		directly			Ste12	GP				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_18_2887_s_193	9744865	( A) Unphosphorylated Kss1 binds directly to Ste12, and to Dig1 and Dig2, thereby stabilizing Dig1/2-Ste12 complexes and potentiating Dig-mediated repression of Ste12.	bind
58366	2	756	5	NULL	NULL	0	NULL	Kss1	GP	unphosphorylated	bind		directly			Dig1	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_18_2887_s_193	9744865	( A) Unphosphorylated Kss1 binds directly to Ste12, and to Dig1 and Dig2, thereby stabilizing Dig1/2-Ste12 complexes and potentiating Dig-mediated repression of Ste12.	bind
58367	3	756	5	NULL	NULL	0	NULL	Kss1	GP	unphosphorylated	bind		directly			Dig2	GP				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_18_2887_s_193	9744865	( A) Unphosphorylated Kss1 binds directly to Ste12, and to Dig1 and Dig2, thereby stabilizing Dig1/2-Ste12 complexes and potentiating Dig-mediated repression of Ste12.	bind
58368	4	756	5	NULL	NULL	0	NULL	statement 1	Process		stabilize					Dig1/2-Ste12 complexes	GP				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_18_2887_s_193	9744865	( A) Unphosphorylated Kss1 binds directly to Ste12, and to Dig1 and Dig2, thereby stabilizing Dig1/2-Ste12 complexes and potentiating Dig-mediated repression of Ste12.	bind
58369	5	756	5	NULL	NULL	0	NULL	statement 2	Process		stabilize					Dig1/2-Ste12 complexes	GP				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_18_2887_s_193	9744865	( A) Unphosphorylated Kss1 binds directly to Ste12, and to Dig1 and Dig2, thereby stabilizing Dig1/2-Ste12 complexes and potentiating Dig-mediated repression of Ste12.	bind
58370	6	756	5	NULL	NULL	0	NULL	statement 3	Process		stabilize					Dig1/2-Ste12 complexes	GP				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_18_2887_s_193	9744865	( A) Unphosphorylated Kss1 binds directly to Ste12, and to Dig1 and Dig2, thereby stabilizing Dig1/2-Ste12 complexes and potentiating Dig-mediated repression of Ste12.	bind
58371	7	756	5	NULL	NULL	0	NULL	Dig	GP		repress					Ste12	GP				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_18_2887_s_193	9744865	( A) Unphosphorylated Kss1 binds directly to Ste12, and to Dig1 and Dig2, thereby stabilizing Dig1/2-Ste12 complexes and potentiating Dig-mediated repression of Ste12.	bind
58372	8	756	5	NULL	NULL	0	NULL	statement 4	Process		potentiate					statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_18_2887_s_193	9744865	( A) Unphosphorylated Kss1 binds directly to Ste12, and to Dig1 and Dig2, thereby stabilizing Dig1/2-Ste12 complexes and potentiating Dig-mediated repression of Ste12.	bind
58373	9	756	5	NULL	NULL	0	NULL	statement 5	Process		potentiate					statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_18_2887_s_193	9744865	( A) Unphosphorylated Kss1 binds directly to Ste12, and to Dig1 and Dig2, thereby stabilizing Dig1/2-Ste12 complexes and potentiating Dig-mediated repression of Ste12.	bind
58374	10	756	5	NULL	NULL	0	NULL	statement 6	Process		potentiate					statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_18_2887_s_193	9744865	( A) Unphosphorylated Kss1 binds directly to Ste12, and to Dig1 and Dig2, thereby stabilizing Dig1/2-Ste12 complexes and potentiating Dig-mediated repression of Ste12.	bind
2039	1	756	6	NULL	NULL	0	NULL	Kss1	GP	unphosphorylated	bind		directly			Ste12	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_18_2887_s_193	9744865	( A) Unphosphorylated Kss1 binds directly to Ste12, and to Dig1 and Dig2, thereby stabilizing Dig1/2-Ste12 complexes and potentiating Dig-mediated repression of Ste12.	bind
2040	2	756	6	NULL	NULL	0	NULL	Kss1	GP	unphosphorylated	bind		directly			Dig1	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_18_2887_s_193	9744865	( A) Unphosphorylated Kss1 binds directly to Ste12, and to Dig1 and Dig2, thereby stabilizing Dig1/2-Ste12 complexes and potentiating Dig-mediated repression of Ste12.	bind
2041	3	756	6	NULL	NULL	0	NULL	Kss1	GP	unphosphorylated	bind		directly			Dig2	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_18_2887_s_193	9744865	( A) Unphosphorylated Kss1 binds directly to Ste12, and to Dig1 and Dig2, thereby stabilizing Dig1/2-Ste12 complexes and potentiating Dig-mediated repression of Ste12.	bind
2042	4	756	6	NULL	NULL	0	NULL	Dig	GP		mediates					Ste12	GP	repression of			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_18_2887_s_193	9744865	( A) Unphosphorylated Kss1 binds directly to Ste12, and to Dig1 and Dig2, thereby stabilizing Dig1/2-Ste12 complexes and potentiating Dig-mediated repression of Ste12.	bind
2043	5	756	6	NULL	NULL	0	NULL	Kss1	GP		potentiates					Statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_18_2887_s_193	9744865	( A) Unphosphorylated Kss1 binds directly to Ste12, and to Dig1 and Dig2, thereby stabilizing Dig1/2-Ste12 complexes and potentiating Dig-mediated repression of Ste12.	bind
2044	6	756	6	NULL	NULL	0	NULL	Kss1	GP		stabilizes					Dig1/2-Ste12 complexes	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_18_2887_s_193	9744865	( A) Unphosphorylated Kss1 binds directly to Ste12, and to Dig1 and Dig2, thereby stabilizing Dig1/2-Ste12 complexes and potentiating Dig-mediated repression of Ste12.	bind
58375	1	757	5	NULL	NULL	0	NULL	RNAP	GP	host	bind					A2b	GP			promoter	NULL		0	NULL	NULL	NULL	gw60_embo_20_21_6060_s_213	11689446	( A) Upon phage infection, the host RNAP binds to promoters A2b and A2c, giving rise to transcription of genes 6 to 1 (see Figure 1), while binding to promoter A3 requires synthesis of protein p4.	bind
58376	2	757	5	NULL	NULL	0	NULL	RNAP	GP	host	bind					A2c	GP			promoter	NULL		0	NULL	NULL	NULL	gw60_embo_20_21_6060_s_213	11689446	( A) Upon phage infection, the host RNAP binds to promoters A2b and A2c, giving rise to transcription of genes 6 to 1 (see Figure 1), while binding to promoter A3 requires synthesis of protein p4.	bind
58377	3	757	5	NULL	NULL	0	NULL	statement 1	Process		occurs upon					phage infection	Process				NULL		0	NULL	NULL	NULL	gw60_embo_20_21_6060_s_213	11689446	( A) Upon phage infection, the host RNAP binds to promoters A2b and A2c, giving rise to transcription of genes 6 to 1 (see Figure 1), while binding to promoter A3 requires synthesis of protein p4.	bind
58378	4	757	5	NULL	NULL	0	NULL	statement 2	Process		occurs upon					phage infection	Process				NULL		0	NULL	NULL	NULL	gw60_embo_20_21_6060_s_213	11689446	( A) Upon phage infection, the host RNAP binds to promoters A2b and A2c, giving rise to transcription of genes 6 to 1 (see Figure 1), while binding to promoter A3 requires synthesis of protein p4.	bind
58379	5	757	5	NULL	NULL	0	NULL	RNAP	GP	host	bind					A3	GP			promoter	NULL		0	NULL	NULL	NULL	gw60_embo_20_21_6060_s_213	11689446	( A) Upon phage infection, the host RNAP binds to promoters A2b and A2c, giving rise to transcription of genes 6 to 1 (see Figure 1), while binding to promoter A3 requires synthesis of protein p4.	bind
58380	6	757	5	NULL	NULL	0	NULL	statement 5	Process		requires					protein p4	GP	synthesis of			NULL		0	NULL	NULL	NULL	gw60_embo_20_21_6060_s_213	11689446	( A) Upon phage infection, the host RNAP binds to promoters A2b and A2c, giving rise to transcription of genes 6 to 1 (see Figure 1), while binding to promoter A3 requires synthesis of protein p4.	bind
2045	1	757	6	NULL	NULL	0	NULL	RNAP	GP		bind					A2b	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_20_21_6060_s_213	11689446	( A) Upon phage infection, the host RNAP binds to promoters A2b and A2c, giving rise to transcription of genes 6 to 1 (see Figure 1), while binding to promoter A3 requires synthesis of protein p4.	bind
2046	2	757	6	NULL	NULL	0	NULL	RNAP	GP		bind					A2c	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_20_21_6060_s_213	11689446	( A) Upon phage infection, the host RNAP binds to promoters A2b and A2c, giving rise to transcription of genes 6 to 1 (see Figure 1), while binding to promoter A3 requires synthesis of protein p4.	bind
2186	3	757	6	NULL	NULL	0	NULL	RNAP	GP		bind					A3	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_20_21_6060_s_213	11689446	( A) Upon phage infection, the host RNAP binds to promoters A2b and A2c, giving rise to transcription of genes 6 to 1 (see Figure 1), while binding to promoter A3 requires synthesis of protein p4.	bind
2187	4	757	6	NULL	NULL	0	NULL	statement 3	GP		requires					protein p4	GP	synthesis of			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_21_6060_s_213	11689446	( A) Upon phage infection, the host RNAP binds to promoters A2b and A2c, giving rise to transcription of genes 6 to 1 (see Figure 1), while binding to promoter A3 requires synthesis of protein p4.	bind
2188	5	757	6	NULL	NULL	0	NULL	statement 1	Process		results in					genes 6 to 1	GP	transcription of 			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_21_6060_s_213	11689446	( A) Upon phage infection, the host RNAP binds to promoters A2b and A2c, giving rise to transcription of genes 6 to 1 (see Figure 1), while binding to promoter A3 requires synthesis of protein p4.	bind
2189	6	757	6	NULL	NULL	0	NULL	statement 2	Process		results in					genes 6 to 1	GP	transcription of 			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_21_6060_s_213	11689446	( A) Upon phage infection, the host RNAP binds to promoters A2b and A2c, giving rise to transcription of genes 6 to 1 (see Figure 1), while binding to promoter A3 requires synthesis of protein p4.	bind
58381	1	759	5	NULL	NULL	0	NULL	Asf1	GP		bind					histone H3/H4 complex	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_102_17_5975_s_131	15840725	( a) V94R, D54R, and R108E are involved in the binding of Asf1 to the histone H3/H4 complex.	bind
2047	1	759	6	NULL	NULL	0	NULL	Asf1	GP		bind					histone H3/H4 complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_17_5975_s_131	15840725	( a) V94R, D54R, and R108E are involved in the binding of Asf1 to the histone H3/H4 complex.	bind
2048	2	759	6	NULL	NULL	0	NULL		AminoAcid		is involved in			V94R		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_17_5975_s_131	15840725	( a) V94R, D54R, and R108E are involved in the binding of Asf1 to the histone H3/H4 complex.	bind
2049	3	759	6	NULL	NULL	0	NULL		AminoAcid		is involved in			D54R		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_17_5975_s_131	15840725	( a) V94R, D54R, and R108E are involved in the binding of Asf1 to the histone H3/H4 complex.	bind
52124	4	759	6	NULL	NULL	0	NULL		AminoAcid		is involved in			R108E		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_17_5975_s_131	15840725	( a) V94R, D54R, and R108E are involved in the binding of Asf1 to the histone H3/H4 complex.	bind
58382	1	761	5	NULL	NULL	0	NULL	Vancomycin	GP		bind					peptidoglycan	CellComponent	growing	D-Ala-D-Ala moiety		NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_20_11028_s_18	10500118	( A) Vancomycin binds the D-Ala-D-Ala moiety of the growing peptidoglycan and sterically occludes the transglycosylation and transpeptidation steps of cell-wall assembly.	bind
58383	2	761	5	NULL	NULL	0	NULL	statement 1	Process		occlude		sterically			cell-wall assembly	Process	transglycosylation step of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_20_11028_s_18	10500118	( A) Vancomycin binds the D-Ala-D-Ala moiety of the growing peptidoglycan and sterically occludes the transglycosylation and transpeptidation steps of cell-wall assembly.	bind
58384	3	761	5	NULL	NULL	0	NULL	statement 1	Process		occlude		sterically			cell-wall assembly	Process	transpeptidation step of			NULL		0	NULL	NULL	NULL	gw60_pnas_96_20_11028_s_18	10500118	( A) Vancomycin binds the D-Ala-D-Ala moiety of the growing peptidoglycan and sterically occludes the transglycosylation and transpeptidation steps of cell-wall assembly.	bind
2050	1	761	6	NULL	NULL	0	NULL	Vancomycin	GP		bind					peptidoglycan	CellComponent		D-Ala-D-Ala moiety 		NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_20_11028_s_18	10500118	( A) Vancomycin binds the D-Ala-D-Ala moiety of the growing peptidoglycan and sterically occludes the transglycosylation and transpeptidation steps of cell-wall assembly.	bind
52125	2	761	6	NULL	NULL	0	NULL	statement 1	Process		occludes		sterically			cell-wall 	CellComponent	transglycosylation of;;assembly of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_20_11028_s_18	10500118	( A) Vancomycin binds the D-Ala-D-Ala moiety of the growing peptidoglycan and sterically occludes the transglycosylation and transpeptidation steps of cell-wall assembly.	bind
52126	3	761	6	NULL	NULL	0	NULL	statement 1	Process		occludes		sterically			cell-wall 	CellComponent	transpeptidation of;;assembly of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_20_11028_s_18	10500118	( A) Vancomycin binds the D-Ala-D-Ala moiety of the growing peptidoglycan and sterically occludes the transglycosylation and transpeptidation steps of cell-wall assembly.	bind
58385	1	763	5	NULL	NULL	0	NULL	VEGF-D	GP		bind					VEGFR-3	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_32_11658_s_160	15289610	( A) VEGFR-3 neutralizing antibody treatment, which blocks VEGF-D binding to VEGFR-3,  specifically suppressed lymphangiogenesis, whereas angiogenesis was unaffected.	bind
58386	2	763	5	NULL	NULL	0	NULL	VEGFR-3 neutralizing antibody	GP		blocks					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_101_32_11658_s_160	15289610	( A) VEGFR-3 neutralizing antibody treatment, which blocks VEGF-D binding to VEGFR-3,  specifically suppressed lymphangiogenesis, whereas angiogenesis was unaffected.	bind
58387	3	763	5	NULL	NULL	0	NULL	statement 2	Process		suppress		specifically			lymphangiogenesis	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_101_32_11658_s_160	15289610	( A) VEGFR-3 neutralizing antibody treatment, which blocks VEGF-D binding to VEGFR-3,  specifically suppressed lymphangiogenesis, whereas angiogenesis was unaffected.	bind
58388	4	763	5	NULL	NULL	0	NULL	statement 2	Process		does not affect					angiogenesis	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_101_32_11658_s_160	15289610	( A) VEGFR-3 neutralizing antibody treatment, which blocks VEGF-D binding to VEGFR-3,  specifically suppressed lymphangiogenesis, whereas angiogenesis was unaffected.	bind
2051	1	763	6	NULL	NULL	0	NULL	VEGF-D	GP		bind					VEGFR-3	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_32_11658_s_160	15289610	( A) VEGFR-3 neutralizing antibody treatment, which blocks VEGF-D binding to VEGFR-3,  specifically suppressed lymphangiogenesis, whereas angiogenesis was unaffected.	bind
2052	2	763	6	NULL	NULL	0	NULL	VEGFR-3	GP		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_32_11658_s_160	15289610	( A) VEGFR-3 neutralizing antibody treatment, which blocks VEGF-D binding to VEGFR-3,  specifically suppressed lymphangiogenesis, whereas angiogenesis was unaffected.	bind
2053	3	763	6	NULL	NULL	0	NULL	VEGFR-3	GP		suppressed		specifically			lymphangiogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_32_11658_s_160	15289610	( A) VEGFR-3 neutralizing antibody treatment, which blocks VEGF-D binding to VEGFR-3,  specifically suppressed lymphangiogenesis, whereas angiogenesis was unaffected.	bind
2054	4	763	6	NULL	NULL	0	NULL	VEGFR-3	GP		has no effect					angiogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_32_11658_s_160	15289610	( A) VEGFR-3 neutralizing antibody treatment, which blocks VEGF-D binding to VEGFR-3,  specifically suppressed lymphangiogenesis, whereas angiogenesis was unaffected.	bind
58389	1	764	5	NULL	NULL	0	NULL	radixin			bind			FERM domain		ICAM-2 peptide	GP				NULL		0	NULL	NULL	NULL	gw60_embo_22_3_502_s_46	12554651	( A) Views of the radixin FERM domain bound to the ICAM-2 peptide by ribbon representations.	bind
2055	1	764	6	NULL	NULL	0	NULL	radixin	GP		bind			FERM domain		ICAM-2 peptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_3_502_s_46	12554651	( A) Views of the radixin FERM domain bound to the ICAM-2 peptide by ribbon representations.	bind
58390	1	765	5	NULL	NULL	0	NULL	Vinculin	GP		bind					F-actin	GP				NULL		0	NULL	NULL	NULL	gw60_embo_18_21_5853_s_167	10545097	( A) Vinculin binds to F-actin in the presence of IpaA in a co-sedimentation assay.	bind
58391	2	765	5	NULL	NULL	0	NULL	statement 1	Process		in the presence of					IpaA	GP				NULL		0	NULL	NULL	NULL	gw60_embo_18_21_5853_s_167	10545097	( A) Vinculin binds to F-actin in the presence of IpaA in a co-sedimentation assay.	bind
2056	1	765	6	NULL	NULL	0	NULL	vinculin	GP		bind					F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_5853_s_167	10545097	( A) Vinculin binds to F-actin in the presence of IpaA in a co-sedimentation assay.	bind
2057	2	765	6	NULL	NULL	0	NULL	statement 1	Process		occurs in presence of 					IpaA	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_5853_s_167	10545097	( A) Vinculin binds to F-actin in the presence of IpaA in a co-sedimentation assay.	bind
58392	1	773	5	NULL	NULL	0	NULL	Gcn5	GP	yeast	bind					AcCoA	GP				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_70_0_81_s_223	11395403	( A) yeast Gcn5 ( 138) and ( B) yeast HAT1 bound to acetyl-CoA (AcCoA) ( 78).	bind
58393	2	773	5	NULL	NULL	0	NULL	HAT1	GP	yeast	bind					AcCoA	GP				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_70_0_81_s_223	11395403	( A) yeast Gcn5 ( 138) and ( B) yeast HAT1 bound to acetyl-CoA (AcCoA) ( 78).	bind
58394	3	773	5	NULL	NULL	0	NULL	AcCoA	GP		is					acetyl-CoA	GP				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_70_0_81_s_223	11395403	( A) yeast Gcn5 ( 138) and ( B) yeast HAT1 bound to acetyl-CoA (AcCoA) ( 78).	bind
2058	1	773	6	NULL	NULL	0	NULL	Gcn5	GP	yeast	bind					acetyl-CoA 	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_70_0_81_s_223	11395403	( A) yeast Gcn5 ( 138) and ( B) yeast HAT1 bound to acetyl-CoA (AcCoA) ( 78).	bind
2059	2	773	6	NULL	NULL	0	NULL	HAT1	GP	Yeast	bind					acetyl-CoA 	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_70_0_81_s_223	11395403	( A) yeast Gcn5 ( 138) and ( B) yeast HAT1 bound to acetyl-CoA (AcCoA) ( 78).	bind
52127	3	773	6	NULL	NULL	0	NULL	AcCoA	Chemical		is					acetyl-CoA	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_70_0_81_s_223	11395403	( A) yeast Gcn5 ( 138) and ( B) yeast HAT1 bound to acetyl-CoA (AcCoA) ( 78).	bind
58395	1	774	5	NULL	NULL	0	NULL	guanylyltransferase	GP	yeast	bind					CTD	AminoAcid	phosphorylated			NULL		0	NULL	NULL	NULL	gw60_genesdev_11_24_3306_s_226	9407024	( A) Yeast guanylyltransferase, Ceg-1, methyltransferase, and Abd-1 bind to the phosphorylated CTD.	bind
58396	2	774	5	NULL	NULL	0	NULL	Ceg-1	GP	yeast	bind					CTD	AminoAcid	phosphorylated			NULL		0	NULL	NULL	NULL	gw60_genesdev_11_24_3306_s_226	9407024	( A) Yeast guanylyltransferase, Ceg-1, methyltransferase, and Abd-1 bind to the phosphorylated CTD.	bind
58397	3	774	5	NULL	NULL	0	NULL	methyltransferase	GP	yeast	bind					CTD	AminoAcid	phosphorylated			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_24_3306_s_226	9407024	( A) Yeast guanylyltransferase, Ceg-1, methyltransferase, and Abd-1 bind to the phosphorylated CTD.	bind
2060	1	774	6	NULL	NULL	0	NULL	guanylyltransferase	GP	Yeast	bind						AminoAcid	phosphorylated	CTD		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_24_3306_s_226	9407024	( A) Yeast guanylyltransferase, Ceg-1, methyltransferase, and Abd-1 bind to the phosphorylated CTD.	bind
2061	2	774	6	NULL	NULL	0	NULL	Ceg-1	GP	Yeast	bind						AminoAcid	phosphorylated	CTD		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_24_3306_s_226	9407024	( A) Yeast guanylyltransferase, Ceg-1, methyltransferase, and Abd-1 bind to the phosphorylated CTD.	bind
2062	3	774	6	NULL	NULL	0	NULL	methyltransferase	GP	Yeast	bind						AminoAcid	phosphorylated	CTD		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_24_3306_s_226	9407024	( A) Yeast guanylyltransferase, Ceg-1, methyltransferase, and Abd-1 bind to the phosphorylated CTD.	bind
2063	4	774	6	NULL	NULL	0	NULL	Abd-1	GP	Yeast	bind						AminoAcid	phosphorylated	CTD		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_24_3306_s_226	9407024	( A) Yeast guanylyltransferase, Ceg-1, methyltransferase, and Abd-1 bind to the phosphorylated CTD.	bind
58398	1	776	5	NULL	NULL	0	NULL	AP-2	GP		bind					synaptotagmin I	GP		C2B domain		NULL		0	NULL	NULL	NULL	gw60_science_285_5431_1268_s_33	10455054	( A) YXX  peptides stimulate AP-2 binding to the C2B domain of synaptotagmin I.	bind
58399	2	776	5	NULL	NULL	0	NULL	YXX peptides	AminoAcid		stimulates					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_science_285_5431_1268_s_33	10455054	( A) YXX  peptides stimulate AP-2 binding to the C2B domain of synaptotagmin I.	bind
2064	1	776	6	NULL	NULL	0	NULL	AP2	GP		bind					synaptotagmin I	GP		C2B domain		NULL		NULL	NULL	NULL	NULL	gw60_science_285_5431_1268_s_33	10455054	( A) YXX  peptides stimulate AP-2 binding to the C2B domain of synaptotagmin I.	bind
2065	2	776	6	NULL	NULL	0	NULL	YXX peptides	GP		stimulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_285_5431_1268_s_33	10455054	( A) YXX  peptides stimulate AP-2 binding to the C2B domain of synaptotagmin I.	bind
58400	1	777	5	NULL	NULL	0	NULL	YY1	GP		bind					CFTR	GP			CArG elements	NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_16_5271_s_375	16170155	( A) YY1 binding to CFTR-CArG elements.	bind
2066	1	777	6	NULL	NULL	0	NULL	YY1	GP		bind					CFTR	GP			CArG element	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_16_5271_s_375	16170155	( A) YY1 binding to CFTR-CArG elements.	bind
58401	1	778	5	NULL	NULL	0	NULL	Z-DNA	NucleicAcid		bind					yabZalphaE3L	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_40_14367_s_103	15448208	( A) Z-DNA binding of yabZalphaE3L as measured by CD.	bind
2067	1	778	6	NULL	NULL	0	NULL	Z-DNA	NucleicAcid		bind						AminoAcid		yabZalphaE3L		NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_40_14367_s_103	15448208	( A) Z-DNA binding of yabZalphaE3L as measured by CD.	bind
58402	1	779	5	NULL	NULL	0	NULL	ZO-3	GP		bind					ZO-1	GP				NULL	MDCK cell extracts	0	NULL	NULL	NULL	gw60_cellbiol_141_1_199_s_135	9531559	( a) ZO-3 binds  ZO-1 and ZO-2 from MDCK  cell extracts.	bind
58403	2	779	5	NULL	NULL	0	NULL	ZO-3	GP		bind					ZO-2	GP				NULL	MDCK cell extracts	NULL	NULL	NULL	NULL	gw60_cellbiol_141_1_199_s_135	9531559	( a) ZO-3 binds  ZO-1 and ZO-2 from MDCK  cell extracts.	bind
2068	1	779	6	NULL	NULL	0	NULL	ZO-3	GP		bind					ZO-1	GP				NULL	MDCK cell extracts	NULL	NULL	NULL	NULL	gw60_cellbiol_141_1_199_s_135	9531559	( a) ZO-3 binds  ZO-1 and ZO-2 from MDCK  cell extracts.	bind
2069	2	779	6	NULL	NULL	0	NULL	ZO-3	GP		bind					ZO-2	GP				NULL	MDCK cell extracts	NULL	NULL	NULL	NULL	gw60_cellbiol_141_1_199_s_135	9531559	( a) ZO-3 binds  ZO-1 and ZO-2 from MDCK  cell extracts.	bind
58404	1	780	5	NULL	NULL	0	NULL	[gamma-32]GTP-V14RhoA	GP		bind		specifically			RhoGAP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_103_11_1561_s_231	10359565	( a) [gamma-32]GTP-V14RhoA specifically binds RhoGAP (positive control) and GST-IL-1Rcd, but not the negative controls GST and BSA.	bind
58405	2	780	5	NULL	NULL	0	NULL	[gamma-32]GTP-V14RhoA	GP		bind		specifically			GST-IL-1Rcd	GP				NULL		0	NULL	NULL	NULL	gw60_jclininvest_103_11_1561_s_231	10359565	( a) [gamma-32]GTP-V14RhoA specifically binds RhoGAP (positive control) and GST-IL-1Rcd, but not the negative controls GST and BSA.	bind
58406	3	780	5	NULL	NULL	0	NULL	[gamma-32]GTP-V14RhoA	GP		does not bind					GST	Chemical				NULL		0	NULL	NULL	NULL	gw60_jclininvest_103_11_1561_s_231	10359565	( a) [gamma-32]GTP-V14RhoA specifically binds RhoGAP (positive control) and GST-IL-1Rcd, but not the negative controls GST and BSA.	bind
58407	4	780	5	NULL	NULL	0	NULL	[gamma-32]GTP-V14RhoA	GP		does not bind					BSA	Chemical				NULL		0	NULL	NULL	NULL	gw60_jclininvest_103_11_1561_s_231	10359565	( a) [gamma-32]GTP-V14RhoA specifically binds RhoGAP (positive control) and GST-IL-1Rcd, but not the negative controls GST and BSA.	bind
2070	1	780	6	NULL	NULL	0	NULL	GTP-V14RhoA	GP		bind		specifically			RhoGAP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_103_11_1561_s_231	10359565	( a) [gamma-32]GTP-V14RhoA specifically binds RhoGAP (positive control) and GST-IL-1Rcd, but not the negative controls GST and BSA.	bind
2071	2	780	6	NULL	NULL	0	NULL	GTP-V14RhoA	GP		bind		specifically			GST-IL-1Rcd	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_103_11_1561_s_231	10359565	( a) [gamma-32]GTP-V14RhoA specifically binds RhoGAP (positive control) and GST-IL-1Rcd, but not the negative controls GST and BSA.	bind
58408	1	781	5	NULL	NULL	0	NULL	cTnC	GP		bind					cTnI	GP		(1-80)DD		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_24_16681_s_86	10358006	( A),  cTnC  bound to cTnI-(1-80)DD ( B), and free  cTnC  ( C).	bind
2074	1	781	6	NULL	NULL	0	NULL	cTnC	GP		bind					cTnI	GP		(1-80)DD		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_24_16681_s_86	10358006	( A),  cTnC  bound to cTnI-(1-80)DD ( B), and free  cTnC  ( C).	bind
2075	2	781	6	NULL	NULL	0	NULL	cTnC	GP		bind					cTnC	GP	free			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_24_16681_s_86	10358006	( A),  cTnC  bound to cTnI-(1-80)DD ( B), and free  cTnC  ( C).	bind
58409	1	796	5	NULL	NULL	0	NULL	SCS	GP	pig	is specific to					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_16_11058_s_185	16481318	( A), GDP bound to pig GTP-specific SCS ( gray) ( B), and ATP bound to glycinamide ribonucleotide transformylase ( gray) (PDB identifier 1kj8) (  ) ( C).	bind
58410	2	796	5	NULL	NULL	0	NULL	GDP	Chemical		bind					statement 1	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_16_11058_s_185	16481318	( A), GDP bound to pig GTP-specific SCS ( gray) ( B), and ATP bound to glycinamide ribonucleotide transformylase ( gray) (PDB identifier 1kj8) (  ) ( C).	bind
58411	3	796	5	NULL	NULL	0	NULL	ATP	Chemical		bind					glycinamide ribonucleotide transformylase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_16_11058_s_185	16481318	( A), GDP bound to pig GTP-specific SCS ( gray) ( B), and ATP bound to glycinamide ribonucleotide transformylase ( gray) (PDB identifier 1kj8) (  ) ( C).	bind
2076	1	796	6	NULL	NULL	0	NULL	GDP	Chemical		bind					SCS	GP	pig;; GTP-specific			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_16_11058_s_185	16481318	( A), GDP bound to pig GTP-specific SCS ( gray) ( B), and ATP bound to glycinamide ribonucleotide transformylase ( gray) (PDB identifier 1kj8) (  ) ( C).	bind
2077	2	796	6	NULL	NULL	0	NULL	ATP	Chemical		bind					glycinamide ribonucleotide transformylase	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_16_11058_s_185	16481318	( A), GDP bound to pig GTP-specific SCS ( gray) ( B), and ATP bound to glycinamide ribonucleotide transformylase ( gray) (PDB identifier 1kj8) (  ) ( C).	bind
63	1	801	6	NULL	NULL	0	NULL	N4BP2	NULL		bind	NULL				GST-Nedd4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2897_s_133	11717310	( A), N4BP2 ( B), and N4BP3 and KIAA0341 ( C) each bind to GST-Nedd4 ( lane 2 in each panel) and GST-Nedd4:N ( lane 3 in each panel) equally well, but show minimal binding to GST-Nedd4:C ( lane 4 in each panel) and GST-E6AP ( lane 6 in each panel) and no binding to GST ( lane 5 in each panel).	bind
64	2	801	6	NULL	NULL	0	NULL	N4BP2	NULL		bind	NULL				GST-Nedd4:N	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2897_s_133	11717310	( A), N4BP2 ( B), and N4BP3 and KIAA0341 ( C) each bind to GST-Nedd4 ( lane 2 in each panel) and GST-Nedd4:N ( lane 3 in each panel) equally well, but show minimal binding to GST-Nedd4:C ( lane 4 in each panel) and GST-E6AP ( lane 6 in each panel) and no binding to GST ( lane 5 in each panel).	bind
65	3	801	6	NULL	NULL	0	NULL	N4BP3	NULL		bind	NULL				GST-Nedd4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2897_s_133	11717310	( A), N4BP2 ( B), and N4BP3 and KIAA0341 ( C) each bind to GST-Nedd4 ( lane 2 in each panel) and GST-Nedd4:N ( lane 3 in each panel) equally well, but show minimal binding to GST-Nedd4:C ( lane 4 in each panel) and GST-E6AP ( lane 6 in each panel) and no binding to GST ( lane 5 in each panel).	bind
66	4	801	6	NULL	NULL	0	NULL	N4BP3	NULL		bind	NULL				GST-Nedd4:N	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2897_s_133	11717310	( A), N4BP2 ( B), and N4BP3 and KIAA0341 ( C) each bind to GST-Nedd4 ( lane 2 in each panel) and GST-Nedd4:N ( lane 3 in each panel) equally well, but show minimal binding to GST-Nedd4:C ( lane 4 in each panel) and GST-E6AP ( lane 6 in each panel) and no binding to GST ( lane 5 in each panel).	bind
67	5	801	6	NULL	NULL	0	NULL	KIAA0341	NULL		bind	NULL				GST-Nedd4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2897_s_133	11717310	( A), N4BP2 ( B), and N4BP3 and KIAA0341 ( C) each bind to GST-Nedd4 ( lane 2 in each panel) and GST-Nedd4:N ( lane 3 in each panel) equally well, but show minimal binding to GST-Nedd4:C ( lane 4 in each panel) and GST-E6AP ( lane 6 in each panel) and no binding to GST ( lane 5 in each panel).	bind
68	6	801	6	NULL	NULL	0	NULL	KIAA0341	NULL		bind	NULL				GST-Nedd4:N	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2897_s_133	11717310	( A), N4BP2 ( B), and N4BP3 and KIAA0341 ( C) each bind to GST-Nedd4 ( lane 2 in each panel) and GST-Nedd4:N ( lane 3 in each panel) equally well, but show minimal binding to GST-Nedd4:C ( lane 4 in each panel) and GST-E6AP ( lane 6 in each panel) and no binding to GST ( lane 5 in each panel).	bind
69	7	801	6	NULL	NULL	0	NULL	N4BP2	NULL		bind	NULL	minimal			GST-Nedd4:C	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2897_s_133	11717310	( A), N4BP2 ( B), and N4BP3 and KIAA0341 ( C) each bind to GST-Nedd4 ( lane 2 in each panel) and GST-Nedd4:N ( lane 3 in each panel) equally well, but show minimal binding to GST-Nedd4:C ( lane 4 in each panel) and GST-E6AP ( lane 6 in each panel) and no binding to GST ( lane 5 in each panel).	bind
70	8	801	6	NULL	NULL	0	NULL	N4BP2	NULL		bind	NULL	minimal			GST-E6AP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2897_s_133	11717310	( A), N4BP2 ( B), and N4BP3 and KIAA0341 ( C) each bind to GST-Nedd4 ( lane 2 in each panel) and GST-Nedd4:N ( lane 3 in each panel) equally well, but show minimal binding to GST-Nedd4:C ( lane 4 in each panel) and GST-E6AP ( lane 6 in each panel) and no binding to GST ( lane 5 in each panel).	bind
71	9	801	6	NULL	NULL	0	NULL	N4BP3	NULL		bind	NULL	minimal			GST-Nedd4:C	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2897_s_133	11717310	( A), N4BP2 ( B), and N4BP3 and KIAA0341 ( C) each bind to GST-Nedd4 ( lane 2 in each panel) and GST-Nedd4:N ( lane 3 in each panel) equally well, but show minimal binding to GST-Nedd4:C ( lane 4 in each panel) and GST-E6AP ( lane 6 in each panel) and no binding to GST ( lane 5 in each panel).	bind
72	10	801	6	NULL	NULL	0	NULL	N4BP3	NULL		bind	NULL	minimal			GST-E6AP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2897_s_133	11717310	( A), N4BP2 ( B), and N4BP3 and KIAA0341 ( C) each bind to GST-Nedd4 ( lane 2 in each panel) and GST-Nedd4:N ( lane 3 in each panel) equally well, but show minimal binding to GST-Nedd4:C ( lane 4 in each panel) and GST-E6AP ( lane 6 in each panel) and no binding to GST ( lane 5 in each panel).	bind
73	11	801	6	NULL	NULL	0	NULL	KIAA0341	NULL		bind	NULL	minimal			GST-Nedd4:C	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2897_s_133	11717310	( A), N4BP2 ( B), and N4BP3 and KIAA0341 ( C) each bind to GST-Nedd4 ( lane 2 in each panel) and GST-Nedd4:N ( lane 3 in each panel) equally well, but show minimal binding to GST-Nedd4:C ( lane 4 in each panel) and GST-E6AP ( lane 6 in each panel) and no binding to GST ( lane 5 in each panel).	bind
74	12	801	6	NULL	NULL	0	NULL	KIAA0341	NULL		bind	NULL	minimal			GST-E6AP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2897_s_133	11717310	( A), N4BP2 ( B), and N4BP3 and KIAA0341 ( C) each bind to GST-Nedd4 ( lane 2 in each panel) and GST-Nedd4:N ( lane 3 in each panel) equally well, but show minimal binding to GST-Nedd4:C ( lane 4 in each panel) and GST-E6AP ( lane 6 in each panel) and no binding to GST ( lane 5 in each panel).	bind
75	13	801	6	NULL	NULL	0	NULL	N4BP2	NULL		does not bind	NULL				GST	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2897_s_133	11717310	( A), N4BP2 ( B), and N4BP3 and KIAA0341 ( C) each bind to GST-Nedd4 ( lane 2 in each panel) and GST-Nedd4:N ( lane 3 in each panel) equally well, but show minimal binding to GST-Nedd4:C ( lane 4 in each panel) and GST-E6AP ( lane 6 in each panel) and no binding to GST ( lane 5 in each panel).	bind
76	14	801	6	NULL	NULL	0	NULL	N4BP3	NULL		does not bind	NULL				GST	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2897_s_133	11717310	( A), N4BP2 ( B), and N4BP3 and KIAA0341 ( C) each bind to GST-Nedd4 ( lane 2 in each panel) and GST-Nedd4:N ( lane 3 in each panel) equally well, but show minimal binding to GST-Nedd4:C ( lane 4 in each panel) and GST-E6AP ( lane 6 in each panel) and no binding to GST ( lane 5 in each panel).	bind
77	15	801	6	NULL	NULL	0	NULL	KIAA0341	NULL		does not bind	NULL				GST	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2897_s_133	11717310	( A), N4BP2 ( B), and N4BP3 and KIAA0341 ( C) each bind to GST-Nedd4 ( lane 2 in each panel) and GST-Nedd4:N ( lane 3 in each panel) equally well, but show minimal binding to GST-Nedd4:C ( lane 4 in each panel) and GST-E6AP ( lane 6 in each panel) and no binding to GST ( lane 5 in each panel).	bind
48147	1	801	7	NULL	NULL	0	NULL	N4BP2	GP		bind					GST-Nedd4	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2897_s_133	11717310	( A), N4BP2 ( B), and N4BP3 and KIAA0341 ( C) each bind to GST-Nedd4 ( lane 2 in each panel) and GST-Nedd4:N ( lane 3 in each panel) equally well, but show minimal binding to GST-Nedd4:C ( lane 4 in each panel) and GST-E6AP ( lane 6 in each panel) and no binding to GST ( lane 5 in each panel).	bind
48148	2	801	7	NULL	NULL	0	NULL	 N4BP2	GP		bind					GST-Nedd4:N	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2897_s_133	11717310	( A), N4BP2 ( B), and N4BP3 and KIAA0341 ( C) each bind to GST-Nedd4 ( lane 2 in each panel) and GST-Nedd4:N ( lane 3 in each panel) equally well, but show minimal binding to GST-Nedd4:C ( lane 4 in each panel) and GST-E6AP ( lane 6 in each panel) and no binding to GST ( lane 5 in each panel).	bind
48149	3	801	7	NULL	NULL	0	NULL	N4BP2	GP		bind		minimally			GST-Nedd4:C	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2897_s_133	11717310	( A), N4BP2 ( B), and N4BP3 and KIAA0341 ( C) each bind to GST-Nedd4 ( lane 2 in each panel) and GST-Nedd4:N ( lane 3 in each panel) equally well, but show minimal binding to GST-Nedd4:C ( lane 4 in each panel) and GST-E6AP ( lane 6 in each panel) and no binding to GST ( lane 5 in each panel).	bind
48150	4	801	7	NULL	NULL	0	NULL	N4BP2	GP		bind		minimally			GST-E6AP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2897_s_133	11717310	( A), N4BP2 ( B), and N4BP3 and KIAA0341 ( C) each bind to GST-Nedd4 ( lane 2 in each panel) and GST-Nedd4:N ( lane 3 in each panel) equally well, but show minimal binding to GST-Nedd4:C ( lane 4 in each panel) and GST-E6AP ( lane 6 in each panel) and no binding to GST ( lane 5 in each panel).	bind
48151	5	801	7	NULL	NULL	0	NULL	N4BP2 	GP		does not bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2897_s_133	11717310	( A), N4BP2 ( B), and N4BP3 and KIAA0341 ( C) each bind to GST-Nedd4 ( lane 2 in each panel) and GST-Nedd4:N ( lane 3 in each panel) equally well, but show minimal binding to GST-Nedd4:C ( lane 4 in each panel) and GST-E6AP ( lane 6 in each panel) and no binding to GST ( lane 5 in each panel).	bind
48152	6	801	7	NULL	NULL	0	NULL	N4BP3	GP		bind					GST-Nedd4	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2897_s_133	11717310	( A), N4BP2 ( B), and N4BP3 and KIAA0341 ( C) each bind to GST-Nedd4 ( lane 2 in each panel) and GST-Nedd4:N ( lane 3 in each panel) equally well, but show minimal binding to GST-Nedd4:C ( lane 4 in each panel) and GST-E6AP ( lane 6 in each panel) and no binding to GST ( lane 5 in each panel).	bind
48153	7	801	7	NULL	NULL	0	NULL	N4BP3 	GP		bind					GST-Nedd4:N	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2897_s_133	11717310	( A), N4BP2 ( B), and N4BP3 and KIAA0341 ( C) each bind to GST-Nedd4 ( lane 2 in each panel) and GST-Nedd4:N ( lane 3 in each panel) equally well, but show minimal binding to GST-Nedd4:C ( lane 4 in each panel) and GST-E6AP ( lane 6 in each panel) and no binding to GST ( lane 5 in each panel).	bind
48154	8	801	7	NULL	NULL	0	NULL	N4BP3	GP		bind		minimally			GST-Nedd4:C	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2897_s_133	11717310	( A), N4BP2 ( B), and N4BP3 and KIAA0341 ( C) each bind to GST-Nedd4 ( lane 2 in each panel) and GST-Nedd4:N ( lane 3 in each panel) equally well, but show minimal binding to GST-Nedd4:C ( lane 4 in each panel) and GST-E6AP ( lane 6 in each panel) and no binding to GST ( lane 5 in each panel).	bind
48155	9	801	7	NULL	NULL	0	NULL	N4BP3	GP		bind		minimally			GST-E6AP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2897_s_133	11717310	( A), N4BP2 ( B), and N4BP3 and KIAA0341 ( C) each bind to GST-Nedd4 ( lane 2 in each panel) and GST-Nedd4:N ( lane 3 in each panel) equally well, but show minimal binding to GST-Nedd4:C ( lane 4 in each panel) and GST-E6AP ( lane 6 in each panel) and no binding to GST ( lane 5 in each panel).	bind
48156	10	801	7	NULL	NULL	0	NULL	N4BP3	GP		does not bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2897_s_133	11717310	( A), N4BP2 ( B), and N4BP3 and KIAA0341 ( C) each bind to GST-Nedd4 ( lane 2 in each panel) and GST-Nedd4:N ( lane 3 in each panel) equally well, but show minimal binding to GST-Nedd4:C ( lane 4 in each panel) and GST-E6AP ( lane 6 in each panel) and no binding to GST ( lane 5 in each panel).	bind
48157	11	801	7	NULL	NULL	0	NULL	KIAA0341	Chemical		bind					GST-Nedd4	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2897_s_133	11717310	( A), N4BP2 ( B), and N4BP3 and KIAA0341 ( C) each bind to GST-Nedd4 ( lane 2 in each panel) and GST-Nedd4:N ( lane 3 in each panel) equally well, but show minimal binding to GST-Nedd4:C ( lane 4 in each panel) and GST-E6AP ( lane 6 in each panel) and no binding to GST ( lane 5 in each panel).	bind
48158	12	801	7	NULL	NULL	0	NULL	KIAA0341	Chemical		bind					GST-Nedd4:N	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2897_s_133	11717310	( A), N4BP2 ( B), and N4BP3 and KIAA0341 ( C) each bind to GST-Nedd4 ( lane 2 in each panel) and GST-Nedd4:N ( lane 3 in each panel) equally well, but show minimal binding to GST-Nedd4:C ( lane 4 in each panel) and GST-E6AP ( lane 6 in each panel) and no binding to GST ( lane 5 in each panel).	bind
48159	13	801	7	NULL	NULL	0	NULL	KIAA0341	Chemical		bind		minimally			GST-Nedd4:C	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2897_s_133	11717310	( A), N4BP2 ( B), and N4BP3 and KIAA0341 ( C) each bind to GST-Nedd4 ( lane 2 in each panel) and GST-Nedd4:N ( lane 3 in each panel) equally well, but show minimal binding to GST-Nedd4:C ( lane 4 in each panel) and GST-E6AP ( lane 6 in each panel) and no binding to GST ( lane 5 in each panel).	bind
48160	14	801	7	NULL	NULL	0	NULL	KIAA0341	Chemical		bind		minimally			GST-E6AP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2897_s_133	11717310	( A), N4BP2 ( B), and N4BP3 and KIAA0341 ( C) each bind to GST-Nedd4 ( lane 2 in each panel) and GST-Nedd4:N ( lane 3 in each panel) equally well, but show minimal binding to GST-Nedd4:C ( lane 4 in each panel) and GST-E6AP ( lane 6 in each panel) and no binding to GST ( lane 5 in each panel).	bind
48161	15	801	7	NULL	NULL	0	NULL	KIAA0341	Chemical		does not bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2897_s_133	11717310	( A), N4BP2 ( B), and N4BP3 and KIAA0341 ( C) each bind to GST-Nedd4 ( lane 2 in each panel) and GST-Nedd4:N ( lane 3 in each panel) equally well, but show minimal binding to GST-Nedd4:C ( lane 4 in each panel) and GST-E6AP ( lane 6 in each panel) and no binding to GST ( lane 5 in each panel).	bind
78	1	805	6	10	NULL	0	NULL	P2 Glu	NULL		bind	NULL					NULL	variant of	S554A		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_48786_s_181	14514675	( A), P2 Glu ( B), and P4 Glu ( C) are bound to the S554A variant.	bind
79	2	805	6	10	NULL	0	NULL	P4 Glu	NULL		bind	NULL					NULL	variant of	S554A		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_48786_s_181	14514675	( A), P2 Glu ( B), and P4 Glu ( C) are bound to the S554A variant.	bind
48162	1	805	7	NULL	NULL	0	NULL	P2 Glu	GP		bind							variant of	S554A		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_48786_s_181	14514675	( A), P2 Glu ( B), and P4 Glu ( C) are bound to the S554A variant.	bind
48163	2	805	7	NULL	NULL	0	NULL	P4 Glu	GP		bind							variant of	S554A		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_48786_s_181	14514675	( A), P2 Glu ( B), and P4 Glu ( C) are bound to the S554A variant.	bind
80	1	806	6	NULL	NULL	0	NULL	p21	NULL		bind	NULL				p53	NULL				NULL	wild type MEFs	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_42_41028_s_176	12909629	( A), p21 ( B), and Perp ( C) bound by p53 in wild type ( Wt) and p53S18A MEFs 18 h after UV radiation.	bind
81	2	806	6	NULL	NULL	0	NULL	p21	NULL		bind	NULL				p53	NULL				NULL	p53S18A MEFs	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_42_41028_s_176	12909629	( A), p21 ( B), and Perp ( C) bound by p53 in wild type ( Wt) and p53S18A MEFs 18 h after UV radiation.	bind
168	3	806	6	NULL	NULL	0	NULL	Perp	NULL		bind	NULL				p53	NULL				NULL	wild type MEFs	0	NULL	NULL	NULL	gw70_jbiolchem_278_42_41028_s_176	12909629	( A), p21 ( B), and Perp ( C) bound by p53 in wild type ( Wt) and p53S18A MEFs 18 h after UV radiation.	bind
169	4	806	6	NULL	NULL	0	NULL	Perp	NULL		bind	NULL				p53	NULL				NULL	p53S18A MEFs	0	NULL	NULL	NULL	gw70_jbiolchem_278_42_41028_s_176	12909629	( A), p21 ( B), and Perp ( C) bound by p53 in wild type ( Wt) and p53S18A MEFs 18 h after UV radiation.	bind
48164	1	806	7	NULL	NULL	0	NULL	p53	GP		bind					p21	GP				NULL	wild type MEFs	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_42_41028_s_176	12909629	( A), p21 ( B), and Perp ( C) bound by p53 in wild type ( Wt) and p53S18A MEFs 18 h after UV radiation.	bind
48165	2	806	7	NULL	NULL	0	NULL	p53	GP		bind					p21	GP				NULL	 p53S18A MEFs	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_42_41028_s_176	12909629	( A), p21 ( B), and Perp ( C) bound by p53 in wild type ( Wt) and p53S18A MEFs 18 h after UV radiation.	bind
48166	3	806	7	NULL	NULL	0	NULL	p53	GP		bind					Perp	GP				NULL	wild type MEFs	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_42_41028_s_176	12909629	( A), p21 ( B), and Perp ( C) bound by p53 in wild type ( Wt) and p53S18A MEFs 18 h after UV radiation.	bind
48167	4	806	7	NULL	NULL	0	NULL	p53	GP		bind					Perp	GP				NULL	 p53S18A MEFs	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_42_41028_s_176	12909629	( A), p21 ( B), and Perp ( C) bound by p53 in wild type ( Wt) and p53S18A MEFs 18 h after UV radiation.	bind
171	2	807	6	NULL	NULL	0	NULL	RFC	NULL		bind	NULL				PCNA-WCad	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_103_8_2546_s_147	16476998	( A), RFC-PCNA-WCad complex formed in the presence of ATP versus DNA bound with streptavidin ( B), RFC versus PCNA-WCad in the presence of ATPgammaS ( C), and RFC-PCNA-WCad complex formed in the presence of ATPgammaS versus DNA - streptavidin ( D).	bind
172	3	807	6	NULL	NULL	0	NULL	statement 2	NULL		forms a 	NULL				complex	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_103_8_2546_s_147	16476998	( A), RFC-PCNA-WCad complex formed in the presence of ATP versus DNA bound with streptavidin ( B), RFC versus PCNA-WCad in the presence of ATPgammaS ( C), and RFC-PCNA-WCad complex formed in the presence of ATPgammaS versus DNA - streptavidin ( D).	bind
173	4	807	6	NULL	NULL	0	NULL	statement 2	NULL		occurs in presence of	NULL				ATPgammaS	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_103_8_2546_s_147	16476998	( A), RFC-PCNA-WCad complex formed in the presence of ATP versus DNA bound with streptavidin ( B), RFC versus PCNA-WCad in the presence of ATPgammaS ( C), and RFC-PCNA-WCad complex formed in the presence of ATPgammaS versus DNA - streptavidin ( D).	bind
48170	1	807	7	NULL	NULL	0	NULL	RFC-PCNA	GP		forms complex with					WCad	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_8_2546_s_147	16476998	( A), RFC-PCNA-WCad complex formed in the presence of ATP versus DNA bound with streptavidin ( B), RFC versus PCNA-WCad in the presence of ATPgammaS ( C), and RFC-PCNA-WCad complex formed in the presence of ATPgammaS versus DNA - streptavidin ( D).	bind
48171	2	807	7	NULL	NULL	0	NULL	statement 1	Process		in presence of					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_8_2546_s_147	16476998	( A), RFC-PCNA-WCad complex formed in the presence of ATP versus DNA bound with streptavidin ( B), RFC versus PCNA-WCad in the presence of ATPgammaS ( C), and RFC-PCNA-WCad complex formed in the presence of ATPgammaS versus DNA - streptavidin ( D).	bind
48173	4	807	7	NULL	NULL	0	NULL	statement 1	Process		in presence of					ATPgammaS	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_8_2546_s_147	16476998	( A), RFC-PCNA-WCad complex formed in the presence of ATP versus DNA bound with streptavidin ( B), RFC versus PCNA-WCad in the presence of ATPgammaS ( C), and RFC-PCNA-WCad complex formed in the presence of ATPgammaS versus DNA - streptavidin ( D).	bind
57975	5	807	7	NULL	NULL	0	NULL	streptavidin 	Chemical		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_8_2546_s_147	16476998	( A), RFC-PCNA-WCad complex formed in the presence of ATP versus DNA bound with streptavidin ( B), RFC versus PCNA-WCad in the presence of ATPgammaS ( C), and RFC-PCNA-WCad complex formed in the presence of ATPgammaS versus DNA - streptavidin ( D).	bind
57976	3	807	7	NULL	NULL	0	NULL	PCNA	GP		complex with					WCad	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_8_2546_s_147	16476998	( A), RFC-PCNA-WCad complex formed in the presence of ATP versus DNA bound with streptavidin ( B), RFC versus PCNA-WCad in the presence of ATPgammaS ( C), and RFC-PCNA-WCad complex formed in the presence of ATPgammaS versus DNA - streptavidin ( D).	bind
57977	6	807	7	NULL	NULL	0	NULL	statement 3	Process		in the presence of					ATPgammaS	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_8_2546_s_147	16476998	( A), RFC-PCNA-WCad complex formed in the presence of ATP versus DNA bound with streptavidin ( B), RFC versus PCNA-WCad in the presence of ATPgammaS ( C), and RFC-PCNA-WCad complex formed in the presence of ATPgammaS versus DNA - streptavidin ( D).	bind
82	1	810	6	NULL	NULL	0	NULL	HMM	NULL		bind	NULL				F-actin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_15_10989_s_123	10753900	( A); however, the addition of 0.2 muM CaD enhanced the binding of HMM to F-actin ( B).	bind
83	2	810	6	NULL	NULL	0	NULL	CaD	NULL		enhance	NULL				Statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_15_10989_s_123	10753900	( A); however, the addition of 0.2 muM CaD enhanced the binding of HMM to F-actin ( B).	bind
48174	1	810	7	NULL	NULL	0	NULL	HMM	GP		bind					F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_15_10989_s_123	10753900	( A); however, the addition of 0.2 muM CaD enhanced the binding of HMM to F-actin ( B).	bind
48175	2	810	7	NULL	NULL	0	NULL	CaD	Chemical		enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_15_10989_s_123	10753900	( A); however, the addition of 0.2 muM CaD enhanced the binding of HMM to F-actin ( B).	bind
166	1	811	6	NULL	NULL	0	NULL	NPG	NULL		bind	NULL				RSO vesicles	NULL	mutant			NULL		0	NULL	NULL	NULL	gw60_pnas_96_20_11178_s_75	10500150	( A*-E*) Flow dialysis profiles comparing binding of NPG to RSO vesicles containing mutants G115A	bind
50312	2	811	6	10	NULL	0	NULL	RSO vesicles	NULL		contains	NULL					NULL	mutants	G115A		NULL		0	NULL	NULL	NULL	gw60_pnas_96_20_11178_s_75	10500150	( A*-E*) Flow dialysis profiles comparing binding of NPG to RSO vesicles containing mutants G115A	bind
48176	1	811	7	NULL	NULL	0	NULL	NPG	Chemical		bind					RSO vesicles	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_20_11178_s_75	10500150	( A*-E*) Flow dialysis profiles comparing binding of NPG to RSO vesicles containing mutants G115A	bind
50313	2	811	7	NULL	NULL	0	NULL	RSO vesicles	Chemical		contains						AminoAcid	mutants	G115A		NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_20_11178_s_75	10500150	( A*-E*) Flow dialysis profiles comparing binding of NPG to RSO vesicles containing mutants G115A	bind
84	1	813	6	NULL	NULL	0	NULL	ATP	NULL		bind	NULL				JNK1	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_23_11_2185_s_156	15141161	( A, B) The binding affinities of ATP to JNK1 were measured by ITC when pepJIP1 was unbound	bind
48177	1	813	7	NULL	NULL	0	NULL	 ATP	Chemical		bind					JNK1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_11_2185_s_156	15141161	( A, B) The binding affinities of ATP to JNK1 were measured by ITC when pepJIP1 was unbound	bind
86	1	815	6	10	NULL	0	NULL	PIAS1	NULL		interacts with	NULL				SATB2	NULL				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_genesdev_17_24_3048_s_148	14701874	( A,B) PIAS1 interacts with SATB2 in vivo.	bind
48178	1	815	7	NULL	NULL	0	NULL	PIAS1	GP		interacts with					SATB2	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_genesdev_17_24_3048_s_148	14701874	( A,B) PIAS1 interacts with SATB2 in vivo.	bind
87	1	816	6	NULL	NULL	0	NULL	Ephrin-B2	NULL		bind	NULL				EphB-rtk8	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_19_3096_s_130	9765210	( A,C), but only ephrin-B2 can bind to EphB-rtk8 ( B,D).	bind
48179	1	816	7	NULL	NULL	0	NULL	ephrin-B2	GP		bind					 EphB-rtk8	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_19_3096_s_130	9765210	( A,C), but only ephrin-B2 can bind to EphB-rtk8 ( B,D).	bind
88	1	818	6	NULL	NULL	0	NULL	TFIIA	NULL		bind	NULL				TRF2	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_96_9_4791_s_147	10220372	( a- d) Western blot analysis of TFIIA and TFIIB binding to TRF2.	bind
89	2	818	6	NULL	NULL	0	NULL	TFIIB	NULL		bind	NULL				TRF2	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_96_9_4791_s_147	10220372	( a- d) Western blot analysis of TFIIA and TFIIB binding to TRF2.	bind
48180	1	818	7	NULL	NULL	0	NULL	TFIIA 	GP		bind					TRF2	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_9_4791_s_147	10220372	( a- d) Western blot analysis of TFIIA and TFIIB binding to TRF2.	bind
48181	2	818	7	NULL	NULL	0	NULL	TFIIB	GP		bind					TRF2	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_9_4791_s_147	10220372	( a- d) Western blot analysis of TFIIA and TFIIB binding to TRF2.	bind
90	1	819	6	10	NULL	0	NULL	NF-kappaB	NULL		bind	NULL				DNA	NULL			PRD11 site	NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10679_s_67	10485885	( a-c) DSP1 helps NF-kappaB ( a) and p50/p50 ( b), but not p65/p65 ( c), bind to DNA bearing PRD11 sites, and an NRE has no effect on that cooperativity.	bind
91	2	819	6	10	NULL	0	NULL	p50/p50	NULL		bind	NULL				DNA	NULL			PRD11 site	NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10679_s_67	10485885	( a-c) DSP1 helps NF-kappaB ( a) and p50/p50 ( b), but not p65/p65 ( c), bind to DNA bearing PRD11 sites, and an NRE has no effect on that cooperativity.	bind
92	3	819	6	10	NULL	0	NULL	p65/p65	NULL		bind	NULL				DNA	NULL			PRD11	NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10679_s_67	10485885	( a-c) DSP1 helps NF-kappaB ( a) and p50/p50 ( b), but not p65/p65 ( c), bind to DNA bearing PRD11 sites, and an NRE has no effect on that cooperativity.	bind
93	4	819	6	NULL	NULL	0	NULL	DSP1	NULL		helps	NULL				Statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_96_19_10679_s_67	10485885	( a-c) DSP1 helps NF-kappaB ( a) and p50/p50 ( b), but not p65/p65 ( c), bind to DNA bearing PRD11 sites, and an NRE has no effect on that cooperativity.	bind
94	5	819	6	NULL	NULL	0	NULL	DSP1	NULL		helps	NULL				Statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_96_19_10679_s_67	10485885	( a-c) DSP1 helps NF-kappaB ( a) and p50/p50 ( b), but not p65/p65 ( c), bind to DNA bearing PRD11 sites, and an NRE has no effect on that cooperativity.	bind
95	6	819	6	10	NULL	0	NULL		NULL		has no effect on	NULL			NRE	Statement 4	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10679_s_67	10485885	( a-c) DSP1 helps NF-kappaB ( a) and p50/p50 ( b), but not p65/p65 ( c), bind to DNA bearing PRD11 sites, and an NRE has no effect on that cooperativity.	bind
96	7	819	6	10	NULL	0	NULL		NULL		has no effect on	NULL			NRE	Statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10679_s_67	10485885	( a-c) DSP1 helps NF-kappaB ( a) and p50/p50 ( b), but not p65/p65 ( c), bind to DNA bearing PRD11 sites, and an NRE has no effect on that cooperativity.	bind
50314	8	819	6	10	NULL	0	NULL	DSP1	NULL		does not help	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_96_19_10679_s_67	10485885	( a-c) DSP1 helps NF-kappaB ( a) and p50/p50 ( b), but not p65/p65 ( c), bind to DNA bearing PRD11 sites, and an NRE has no effect on that cooperativity.	bind
48182	1	819	7	NULL	NULL	0	NULL	NF-kappaB	GP		bind					DNA	NucleicAcid			PRD11 site	NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10679_s_67	10485885	( a-c) DSP1 helps NF-kappaB ( a) and p50/p50 ( b), but not p65/p65 ( c), bind to DNA bearing PRD11 sites, and an NRE has no effect on that cooperativity.	bind
48183	2	819	7	NULL	NULL	0	NULL	p50/p50	GP		bind					DNA	NucleicAcid			PRD11 site	NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10679_s_67	10485885	( a-c) DSP1 helps NF-kappaB ( a) and p50/p50 ( b), but not p65/p65 ( c), bind to DNA bearing PRD11 sites, and an NRE has no effect on that cooperativity.	bind
48184	3	819	7	NULL	NULL	0	NULL	p65/p65	GP		bind					DNA	NucleicAcid			PRD11 site	NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10679_s_67	10485885	( a-c) DSP1 helps NF-kappaB ( a) and p50/p50 ( b), but not p65/p65 ( c), bind to DNA bearing PRD11 sites, and an NRE has no effect on that cooperativity.	bind
48185	4	819	7	NULL	NULL	0	NULL	DSP1	GP		helps in					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10679_s_67	10485885	( a-c) DSP1 helps NF-kappaB ( a) and p50/p50 ( b), but not p65/p65 ( c), bind to DNA bearing PRD11 sites, and an NRE has no effect on that cooperativity.	bind
48186	5	819	7	NULL	NULL	0	NULL	DSP1	GP		helps in					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10679_s_67	10485885	( a-c) DSP1 helps NF-kappaB ( a) and p50/p50 ( b), but not p65/p65 ( c), bind to DNA bearing PRD11 sites, and an NRE has no effect on that cooperativity.	bind
48187	6	819	7	NULL	NULL	0	NULL	DSP1	GP		does not help					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10679_s_67	10485885	( a-c) DSP1 helps NF-kappaB ( a) and p50/p50 ( b), but not p65/p65 ( c), bind to DNA bearing PRD11 sites, and an NRE has no effect on that cooperativity.	bind
48188	7	819	7	NULL	NULL	0	NULL		GP		has no effect on				NRE	statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10679_s_67	10485885	( a-c) DSP1 helps NF-kappaB ( a) and p50/p50 ( b), but not p65/p65 ( c), bind to DNA bearing PRD11 sites, and an NRE has no effect on that cooperativity.	bind
48189	8	819	7	NULL	NULL	0	NULL		GP		has no effect on				NRE	statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10679_s_67	10485885	( a-c) DSP1 helps NF-kappaB ( a) and p50/p50 ( b), but not p65/p65 ( c), bind to DNA bearing PRD11 sites, and an NRE has no effect on that cooperativity.	bind
97	1	820	6	10	NULL	0	NULL	FGF7	NULL		bind	NULL				FGFR2c 	NULL		S252W		NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_26_14536_s_146	11121055	( A-C) FGF7 binding to FGFR2c (S252W), FGFR2c (P253R), and FGFR2b, respectively.	bind
98	2	820	6	10	NULL	0	NULL	FGF7	NULL		bind	NULL				FGFR2c	NULL		P253R		NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_26_14536_s_146	11121055	( A-C) FGF7 binding to FGFR2c (S252W), FGFR2c (P253R), and FGFR2b, respectively.	bind
99	3	820	6	NULL	NULL	0	NULL	FGF7	NULL		bind	NULL				FGFR2b	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_26_14536_s_146	11121055	( A-C) FGF7 binding to FGFR2c (S252W), FGFR2c (P253R), and FGFR2b, respectively.	bind
48191	1	820	7	NULL	NULL	0	NULL	FGF7	GP		bind					FGFR2c	GP		S252W		NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_26_14536_s_146	11121055	( A-C) FGF7 binding to FGFR2c (S252W), FGFR2c (P253R), and FGFR2b, respectively.	bind
48192	2	820	7	NULL	NULL	0	NULL	FGF7	GP		bind					FGFR2c	GP		P253R		NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_26_14536_s_146	11121055	( A-C) FGF7 binding to FGFR2c (S252W), FGFR2c (P253R), and FGFR2b, respectively.	bind
48193	3	820	7	NULL	NULL	0	NULL	FGF7	GP		bind					FGFR2b	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_26_14536_s_146	11121055	( A-C) FGF7 binding to FGFR2c (S252W), FGFR2c (P253R), and FGFR2b, respectively.	bind
100	1	825	6	10	NULL	0	NULL	MeCP2	NULL		bind	NULL		MBD		DNA	NULL	methylated			NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_20_6603_s_80	16314321	( B -  D) Binding of the MBD of MeCP2 to methylated DNA and four-way junction DNA in the presence  of competitor.	bind
101	2	825	6	NULL	NULL	0	NULL	MeCP2	NULL		bind	NULL		MBD		four-way junction DNA	NULL				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_20_6603_s_80	16314321	( B -  D) Binding of the MBD of MeCP2 to methylated DNA and four-way junction DNA in the presence  of competitor.	bind
48194	1	825	7	NULL	NULL	0	NULL	MeCP2	GP		bind			MBD		 DNA	NucleicAcid	 methylated			NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_20_6603_s_80	16314321	( B -  D) Binding of the MBD of MeCP2 to methylated DNA and four-way junction DNA in the presence  of competitor.	bind
48195	2	825	7	NULL	NULL	0	NULL	MeCP2	GP		bind			MBD		four-way junction DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_20_6603_s_80	16314321	( B -  D) Binding of the MBD of MeCP2 to methylated DNA and four-way junction DNA in the presence  of competitor.	bind
102	1	828	6	NULL	NULL	0	NULL	PSF	NULL		bind	NULL				GAGE6	NULL			promoter fragments	NULL		0	NULL	NULL	NULL	gw70_pnas_102_34_12189_s_93	16079199	( B and  C) Binding of PSF to  GAGE6 promoter fragments.	bind
103	1	830	6	10	NULL	0	NULL	sera	NULL	mouse	bind	NULL				M21 cells	NULL				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_9_5396_s_97	12702756	( B and  C) Flow cytometry histogram showing the binding of mouse sera to human melanoma M21  cells.	bind
50315	2	830	6	10	NULL	0	NULL	M21 cells	NULL		is a type of	NULL				human melanoma cells	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_100_9_5396_s_97	12702756	( B and  C) Flow cytometry histogram showing the binding of mouse sera to human melanoma M21  cells.	bind
48198	1	830	7	NULL	NULL	0	NULL	sera	CellComponent	mouse	bind					M21 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_9_5396_s_97	12702756	( B and  C) Flow cytometry histogram showing the binding of mouse sera to human melanoma M21  cells.	bind
50316	2	830	7	NULL	NULL	0	NULL	M21 cells	Cell		is a type of					human melanoma cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_9_5396_s_97	12702756	( B and  C) Flow cytometry histogram showing the binding of mouse sera to human melanoma M21  cells.	bind
106	1	833	6	10	NULL	0	NULL	Fibrinogen	NULL	Soluble	bind	NULL				293T cell transfectants	NULL				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_10_3679_s_94	15738420	( B and  C) Soluble fibrinogen and PAC-1 IgM binding to 293T cell transfectants in the presence  of Ca2+ (white bars), Mn2+ (gray bars), PT25-2 (hatched bars), or Mn/PT25-2 (black bars).	bind
107	2	833	6	10	NULL	0	NULL	PAC-1 IgM	NULL		bind	NULL				293T cell transfectants	NULL				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_10_3679_s_94	15738420	( B and  C) Soluble fibrinogen and PAC-1 IgM binding to 293T cell transfectants in the presence  of Ca2+ (white bars), Mn2+ (gray bars), PT25-2 (hatched bars), or Mn/PT25-2 (black bars).	bind
48201	1	833	7	NULL	NULL	0	NULL	 fibrinogen	GP	soluble	bind					 293T cell transfectants	Cell				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_10_3679_s_94	15738420	( B and  C) Soluble fibrinogen and PAC-1 IgM binding to 293T cell transfectants in the presence  of Ca2+ (white bars), Mn2+ (gray bars), PT25-2 (hatched bars), or Mn/PT25-2 (black bars).	bind
48202	2	833	7	NULL	NULL	0	NULL	PAC-1 IgM	GP		bind					293T cell transfectants	Cell				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_10_3679_s_94	15738420	( B and  C) Soluble fibrinogen and PAC-1 IgM binding to 293T cell transfectants in the presence  of Ca2+ (white bars), Mn2+ (gray bars), PT25-2 (hatched bars), or Mn/PT25-2 (black bars).	bind
48203	3	833	7	NULL	NULL	0	NULL	statement 1	Process		in the presence of					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_10_3679_s_94	15738420	( B and  C) Soluble fibrinogen and PAC-1 IgM binding to 293T cell transfectants in the presence  of Ca2+ (white bars), Mn2+ (gray bars), PT25-2 (hatched bars), or Mn/PT25-2 (black bars).	bind
48204	4	833	7	NULL	NULL	0	NULL	statement 1	Process		in the presence of					Mn2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_10_3679_s_94	15738420	( B and  C) Soluble fibrinogen and PAC-1 IgM binding to 293T cell transfectants in the presence  of Ca2+ (white bars), Mn2+ (gray bars), PT25-2 (hatched bars), or Mn/PT25-2 (black bars).	bind
48205	5	833	7	NULL	NULL	0	NULL	statement 1	Process		in the presence of					PT25-2	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_10_3679_s_94	15738420	( B and  C) Soluble fibrinogen and PAC-1 IgM binding to 293T cell transfectants in the presence  of Ca2+ (white bars), Mn2+ (gray bars), PT25-2 (hatched bars), or Mn/PT25-2 (black bars).	bind
48206	6	833	7	NULL	NULL	0	NULL	statement 1	Process		in the presence of					Mn/PT25-2	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_10_3679_s_94	15738420	( B and  C) Soluble fibrinogen and PAC-1 IgM binding to 293T cell transfectants in the presence  of Ca2+ (white bars), Mn2+ (gray bars), PT25-2 (hatched bars), or Mn/PT25-2 (black bars).	bind
48207	7	833	7	NULL	NULL	0	NULL	statement 2	Process		in the presence of					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_10_3679_s_94	15738420	( B and  C) Soluble fibrinogen and PAC-1 IgM binding to 293T cell transfectants in the presence  of Ca2+ (white bars), Mn2+ (gray bars), PT25-2 (hatched bars), or Mn/PT25-2 (black bars).	bind
48208	8	833	7	NULL	NULL	0	NULL	statement 2	Process		in the presence of					Mn2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_10_3679_s_94	15738420	( B and  C) Soluble fibrinogen and PAC-1 IgM binding to 293T cell transfectants in the presence  of Ca2+ (white bars), Mn2+ (gray bars), PT25-2 (hatched bars), or Mn/PT25-2 (black bars).	bind
48209	9	833	7	NULL	NULL	0	NULL	statement 2	Process		in the presence of					 PT25-2	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_10_3679_s_94	15738420	( B and  C) Soluble fibrinogen and PAC-1 IgM binding to 293T cell transfectants in the presence  of Ca2+ (white bars), Mn2+ (gray bars), PT25-2 (hatched bars), or Mn/PT25-2 (black bars).	bind
48210	10	833	7	NULL	NULL	0	NULL	statement 2	Process		in the presence of					Mn/PT25-2	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_10_3679_s_94	15738420	( B and  C) Soluble fibrinogen and PAC-1 IgM binding to 293T cell transfectants in the presence  of Ca2+ (white bars), Mn2+ (gray bars), PT25-2 (hatched bars), or Mn/PT25-2 (black bars).	bind
108	1	834	6	NULL	NULL	0	NULL	PABP	NULL		bind	NULL				ARS	NULL				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_210	16356927	( B and  C) UV crosslinking assays of binding of PABP to ARS and poly	bind
109	2	834	6	NULL	NULL	0	NULL	PABP	NULL		bind	NULL				poly	NULL				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_210	16356927	( B and  C) UV crosslinking assays of binding of PABP to ARS and poly	bind
48211	1	834	7	NULL	NULL	0	NULL	PABP	GP		bind					ARS	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_210	16356927	( B and  C) UV crosslinking assays of binding of PABP to ARS and poly	bind
58233	1	836	7	NULL	NULL	0	NULL	Thrombin	GP	biotinylated	cleaves					RACK1	GP	free			NULL		0	NULL	NULL	NULL	gw70_pnas_101_8_2328_s_57	14983009	( B Left)  In vitro Coomassie stain of GST-fusion protein binding of purified RACK1 to glutathione Sepharose  and free RACK1 that has been cleaved from GST by using biotinylated thrombin followed  by clearing with streptavidin beads.	bind
113	1	837	6	10	NULL	0	NULL	MutS	NULL	 E. coli	bind	NULL				G/T mismatch	NULL				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_25_14822_s_48	14634210	( b Middle and  Bottom) AFM surface plots of  E. coli MutS bound to a G/T mismatch and  Taq MutS bound to a 1T-bulge, respectively.	bind
114	2	837	6	10	NULL	0	NULL	MutS	NULL	Taq	bind	NULL				1T-bulge	NULL				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_25_14822_s_48	14634210	( b Middle and  Bottom) AFM surface plots of  E. coli MutS bound to a G/T mismatch and  Taq MutS bound to a 1T-bulge, respectively.	bind
48212	1	837	7	NULL	NULL	0	NULL	MutS	GP	E.coli	bind					G/T mismatch	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_25_14822_s_48	14634210	( b Middle and  Bottom) AFM surface plots of  E. coli MutS bound to a G/T mismatch and  Taq MutS bound to a 1T-bulge, respectively.	bind
48213	2	837	7	NULL	NULL	0	NULL	MutS	GP	Taq	bind					1T-bulge	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_25_14822_s_48	14634210	( b Middle and  Bottom) AFM surface plots of  E. coli MutS bound to a G/T mismatch and  Taq MutS bound to a 1T-bulge, respectively.	bind
115	1	838	6	NULL	NULL	0	NULL	Hh	NULL		bind	NULL				receptor Ptc	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_20_4_399_s_43	16481469	( B'') When Hh binds to its receptor Ptc, Smo becomes phosphorylated by PKA and CKIalpha, Smo levels increase, and it accumulates on the cell surface.	bind
116	2	838	6	NULL	NULL	0	NULL	PKA	NULL		phosphorylates	NULL				Smo	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_20_4_399_s_43	16481469	( B'') When Hh binds to its receptor Ptc, Smo becomes phosphorylated by PKA and CKIalpha, Smo levels increase, and it accumulates on the cell surface.	bind
117	3	838	6	NULL	NULL	0	NULL	CKIalpha	NULL		phosphorylates	NULL				Smo	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_20_4_399_s_43	16481469	( B'') When Hh binds to its receptor Ptc, Smo becomes phosphorylated by PKA and CKIalpha, Smo levels increase, and it accumulates on the cell surface.	bind
118	4	838	6	NULL	NULL	0	NULL	Statement 1	NULL		causes	NULL				Statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_20_4_399_s_43	16481469	( B'') When Hh binds to its receptor Ptc, Smo becomes phosphorylated by PKA and CKIalpha, Smo levels increase, and it accumulates on the cell surface.	bind
119	5	838	6	NULL	NULL	0	NULL	Statement 1	NULL		causes	NULL				Statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_20_4_399_s_43	16481469	( B'') When Hh binds to its receptor Ptc, Smo becomes phosphorylated by PKA and CKIalpha, Smo levels increase, and it accumulates on the cell surface.	bind
120	6	838	6	10	NULL	0	NULL	Statement 2	NULL		increases	NULL				Smo	NULL	 levels of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_20_4_399_s_43	16481469	( B'') When Hh binds to its receptor Ptc, Smo becomes phosphorylated by PKA and CKIalpha, Smo levels increase, and it accumulates on the cell surface.	bind
121	7	838	6	10	NULL	0	NULL	Statement 3	NULL		increases	NULL				Smo	NULL	levels of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_20_4_399_s_43	16481469	( B'') When Hh binds to its receptor Ptc, Smo becomes phosphorylated by PKA and CKIalpha, Smo levels increase, and it accumulates on the cell surface.	bind
50317	8	838	6	10	NULL	0	NULL	Smo	NULL		accumulates on	NULL				cell surface	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_20_4_399_s_43	16481469	( B'') When Hh binds to its receptor Ptc, Smo becomes phosphorylated by PKA and CKIalpha, Smo levels increase, and it accumulates on the cell surface.	bind
50318	9	838	6	10	NULL	0	NULL	statement 6	NULL		leads to	NULL				statement 8	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_20_4_399_s_43	16481469	( B'') When Hh binds to its receptor Ptc, Smo becomes phosphorylated by PKA and CKIalpha, Smo levels increase, and it accumulates on the cell surface.	bind
50319	10	838	6	10	NULL	0	NULL	statement 7	NULL		leads to	NULL				statement 8	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_20_4_399_s_43	16481469	( B'') When Hh binds to its receptor Ptc, Smo becomes phosphorylated by PKA and CKIalpha, Smo levels increase, and it accumulates on the cell surface.	bind
48214	1	838	7	NULL	NULL	0	NULL	Hh 	GP		bind					Ptc receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_20_4_399_s_43	16481469	( B'') When Hh binds to its receptor Ptc, Smo becomes phosphorylated by PKA and CKIalpha, Smo levels increase, and it accumulates on the cell surface.	bind
48215	2	838	7	NULL	NULL	0	NULL	PKA	GP		phosphorylate					Smo	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_20_4_399_s_43	16481469	( B'') When Hh binds to its receptor Ptc, Smo becomes phosphorylated by PKA and CKIalpha, Smo levels increase, and it accumulates on the cell surface.	bind
48216	3	838	7	NULL	NULL	0	NULL	CKIalpha	GP		phosphorylate					Smo	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_20_4_399_s_43	16481469	( B'') When Hh binds to its receptor Ptc, Smo becomes phosphorylated by PKA and CKIalpha, Smo levels increase, and it accumulates on the cell surface.	bind
48217	4	838	7	NULL	NULL	0	NULL	statement 2	Process		occurs after					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_20_4_399_s_43	16481469	( B'') When Hh binds to its receptor Ptc, Smo becomes phosphorylated by PKA and CKIalpha, Smo levels increase, and it accumulates on the cell surface.	bind
48218	5	838	7	NULL	NULL	0	NULL	statement 3	Process		occurs after					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_20_4_399_s_43	16481469	( B'') When Hh binds to its receptor Ptc, Smo becomes phosphorylated by PKA and CKIalpha, Smo levels increase, and it accumulates on the cell surface.	bind
48219	6	838	7	NULL	NULL	0	NULL	statement 2	Process		increase					Smo	GP	levels of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_20_4_399_s_43	16481469	( B'') When Hh binds to its receptor Ptc, Smo becomes phosphorylated by PKA and CKIalpha, Smo levels increase, and it accumulates on the cell surface.	bind
48220	7	838	7	NULL	NULL	0	NULL	statement 3	Process		increase					Smo	GP	levels of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_20_4_399_s_43	16481469	( B'') When Hh binds to its receptor Ptc, Smo becomes phosphorylated by PKA and CKIalpha, Smo levels increase, and it accumulates on the cell surface.	bind
48221	8	838	7	NULL	NULL	0	NULL	Smo	GP		accumulates on					cell surface	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_20_4_399_s_43	16481469	( B'') When Hh binds to its receptor Ptc, Smo becomes phosphorylated by PKA and CKIalpha, Smo levels increase, and it accumulates on the cell surface.	bind
48222	9	838	7	NULL	NULL	0	NULL	statement 6	Process		leads to					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_20_4_399_s_43	16481469	( B'') When Hh binds to its receptor Ptc, Smo becomes phosphorylated by PKA and CKIalpha, Smo levels increase, and it accumulates on the cell surface.	bind
48223	10	838	7	NULL	NULL	0	NULL	statement 7	Process		leads to					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_20_4_399_s_43	16481469	( B'') When Hh binds to its receptor Ptc, Smo becomes phosphorylated by PKA and CKIalpha, Smo levels increase, and it accumulates on the cell surface.	bind
123	1	839	6	NULL	NULL	0	NULL	A30	NULL		bind	NULL				HER3	NULL	cellular			NULL		0	NULL	NULL	NULL	gw70_pnas_100_16_9226_s_152	12874383	( B)  Binding of A30 to cellular HER3 also shows an increase in binding sites on  addition  of hrg ( ), although less pronounced than in solution.	bind
124	2	839	6	10	NULL	0	NULL	Hrg	NULL		increases	NULL				HER3	NULL	binding sites of;;cellular			NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_16_9226_s_152	12874383	( B)  Binding of A30 to cellular HER3 also shows an increase in binding sites on  addition  of hrg ( ), although less pronounced than in solution.	bind
125	3	839	6	NULL	NULL	0	NULL	Statement 1	NULL		causes	NULL				Statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_100_16_9226_s_152	12874383	( B)  Binding of A30 to cellular HER3 also shows an increase in binding sites on  addition  of hrg ( ), although less pronounced than in solution.	bind
48224	1	839	7	NULL	NULL	0	NULL	A30	GP		bind					HER3	GP	cellular			NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_16_9226_s_152	12874383	( B)  Binding of A30 to cellular HER3 also shows an increase in binding sites on  addition  of hrg ( ), although less pronounced than in solution.	bind
48225	2	839	7	NULL	NULL	0	NULL	hrg	GP		increase					HER3	GP	binding sites of;;cellular			NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_16_9226_s_152	12874383	( B)  Binding of A30 to cellular HER3 also shows an increase in binding sites on  addition  of hrg ( ), although less pronounced than in solution.	bind
50320	3	839	7	NULL	NULL	0	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_16_9226_s_152	12874383	( B)  Binding of A30 to cellular HER3 also shows an increase in binding sites on  addition  of hrg ( ), although less pronounced than in solution.	bind
122	1	842	6	10	NULL	0	NULL	iC3b	NULL		bind	NULL				COS cells	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_143_6_1523_s_193	9852148	( B)  Histograms (mean  plus-or-minus  SEM,   n = 3) showing the relative  binding of iC3b to COS cells  expressing CR3 mutants.	bind
50321	2	842	6	10	NULL	0	NULL	COS cells	NULL		express	NULL				CR3	NULL	mutants			NULL		0	NULL	NULL	NULL	gw60_cellbiol_143_6_1523_s_193	9852148	( B)  Histograms (mean  plus-or-minus  SEM,   n = 3) showing the relative  binding of iC3b to COS cells  expressing CR3 mutants.	bind
48226	1	842	7	NULL	NULL	0	NULL	 iC3b	GP		bind					COS cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_143_6_1523_s_193	9852148	( B)  Histograms (mean  plus-or-minus  SEM,   n = 3) showing the relative  binding of iC3b to COS cells  expressing CR3 mutants.	bind
48227	2	842	7	NULL	NULL	0	NULL	COS cells	Cell		express					CR3	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_143_6_1523_s_193	9852148	( B)  Histograms (mean  plus-or-minus  SEM,   n = 3) showing the relative  binding of iC3b to COS cells  expressing CR3 mutants.	bind
126	1	843	6	10	NULL	0	NULL	HMGI-C protein	NULL		bind	NULL				IL-15 oligonucleotide	NULL				NULL	In vitro	NULL	NULL	NULL	NULL	gw60_pnas_98_14_7970_s_159	11427729	( B)  In vitro binding of HMGI-C protein to the IL-15 oligonucleotide competed with 30 ng of HMGI/C recombinant protein alone (lane 2) or in presence of two unrelated oligonucleotides (lanes 3 and 4).	bind
127	2	843	6	10	NULL	0	NULL	HMGI/C	NULL	recombinant	bind	NULL				IL-15 oligonucleotide	NULL				NULL	In vitro	NULL	NULL	NULL	NULL	gw60_pnas_98_14_7970_s_159	11427729	( B)  In vitro binding of HMGI-C protein to the IL-15 oligonucleotide competed with 30 ng of HMGI/C recombinant protein alone (lane 2) or in presence of two unrelated oligonucleotides (lanes 3 and 4).	bind
50322	3	843	6	10	NULL	0	NULL	statement 1	NULL		compete with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_98_14_7970_s_159	11427729	( B)  In vitro binding of HMGI-C protein to the IL-15 oligonucleotide competed with 30 ng of HMGI/C recombinant protein alone (lane 2) or in presence of two unrelated oligonucleotides (lanes 3 and 4).	bind
48228	1	843	7	NULL	NULL	0	NULL	HMGI-C protein	GP		bind					IL-15 oligonucleotide	NucleicAcid				NULL	In vitro	NULL	NULL	NULL	NULL	gw60_pnas_98_14_7970_s_159	11427729	( B)  In vitro binding of HMGI-C protein to the IL-15 oligonucleotide competed with 30 ng of HMGI/C recombinant protein alone (lane 2) or in presence of two unrelated oligonucleotides (lanes 3 and 4).	bind
48229	2	843	7	NULL	NULL	0	NULL	HMGI-C protein	GP	recombinant	bind					 IL-15 oligonucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_14_7970_s_159	11427729	( B)  In vitro binding of HMGI-C protein to the IL-15 oligonucleotide competed with 30 ng of HMGI/C recombinant protein alone (lane 2) or in presence of two unrelated oligonucleotides (lanes 3 and 4).	bind
48230	3	843	7	NULL	NULL	0	NULL	statement 1	Process		compete with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_14_7970_s_159	11427729	( B)  In vitro binding of HMGI-C protein to the IL-15 oligonucleotide competed with 30 ng of HMGI/C recombinant protein alone (lane 2) or in presence of two unrelated oligonucleotides (lanes 3 and 4).	bind
128	1	844	6	NULL	NULL	0	NULL	p14ARF	NULL		bind	NULL				MDM2	NULL				NULL	In vitro	0	NULL	NULL	NULL	gw60_embo_17_17_5001_s_121	9724636	( B)  In vitro binding of p14ARF and MDM2.	bind
48231	1	844	7	NULL	NULL	0	NULL	p14ARF	GP		bind					MDM2	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_17_17_5001_s_121	9724636	( B)  In vitro binding of p14ARF and MDM2.	bind
129	1	845	6	NULL	NULL	0	NULL	CDC25C	NULL		bind	NULL			5' UTR	Dazl	NULL				NULL	In vitro	0	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2479_s_58	11410654	( B)  In vitro binding of the CDC25C 5' UTR to Dazl.	bind
48232	1	845	7	NULL	NULL	0	NULL	CDC25C	GP		bind				5' UTR	Dazl	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2479_s_58	11410654	( B)  In vitro binding of the CDC25C 5' UTR to Dazl.	bind
130	1	848	6	10	NULL	0	NULL	ALEX	NULL	in vitro translated	bind	NULL	specifically			GST - XL	NULL		XL-domain		NULL		NULL	NULL	NULL	NULL	gw60_embo_20_14_3849_s_181	11447126	( B)  In vitro translated ALEX binds specifically to the XL-domain of a GST - XL fusion protein.	bind
50323	2	848	6	10	NULL	0	NULL	GST - XL	NULL		is a type of	NULL				fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_20_14_3849_s_181	11447126	( B)  In vitro translated ALEX binds specifically to the XL-domain of a GST - XL fusion protein.	bind
48233	1	848	7	NULL	NULL	0	NULL	ALEX	GP	In vitro translated	bind		specifically			GST - XL	GP		XL-domain		NULL		NULL	NULL	NULL	NULL	gw60_embo_20_14_3849_s_181	11447126	( B)  In vitro translated ALEX binds specifically to the XL-domain of a GST - XL fusion protein.	bind
48234	2	848	7	NULL	NULL	0	NULL	GST-XL	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_14_3849_s_181	11447126	( B)  In vitro translated ALEX binds specifically to the XL-domain of a GST - XL fusion protein.	bind
131	1	849	6	NULL	NULL	0	NULL	DRIP130	NULL	 In vitro translated	bind	NULL				ESX	NULL		activation domain		NULL		0	NULL	NULL	NULL	gw60_pnas_99_20_12747_s_68	12242338	( B)  In vitro translated DRIP130 binds the ESX activation domain but not its activation-deficient mutant.	bind
132	2	849	6	NULL	NULL	0	NULL	DRIP130	NULL	in vitro translated	does not bind	NULL				ESX	NULL	mutant			NULL		0	NULL	NULL	NULL	gw60_pnas_99_20_12747_s_68	12242338	( B)  In vitro translated DRIP130 binds the ESX activation domain but not its activation-deficient mutant.	bind
48235	1	849	7	NULL	NULL	0	NULL	DRIP130	GP	In vitro translated	bind					ESX	GP		activation domain		NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_20_12747_s_68	12242338	( B)  In vitro translated DRIP130 binds the ESX activation domain but not its activation-deficient mutant.	bind
48236	2	849	7	NULL	NULL	0	NULL	DRIP130	GP	In vitro translated	does not bind					ESX	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_20_12747_s_68	12242338	( B)  In vitro translated DRIP130 binds the ESX activation domain but not its activation-deficient mutant.	bind
133	1	850	6	NULL	NULL	0	NULL	MDM2	NULL	in vitro translated	bind	NULL				GST-Sp1	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_98_5_2211_s_102	11226218	( B)  In vitro-translated MDM2 binds to GST-Sp1.	bind
48237	1	850	7	NULL	NULL	0	NULL	MDM2	GP	In vitro-translated	bind					GST-Sp1	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_5_2211_s_102	11226218	( B)  In vitro-translated MDM2 binds to GST-Sp1.	bind
134	1	851	6	NULL	NULL	0	NULL	K562 cells	NULL	PMA-treated	inhibits	NULL				CS-A	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_5_1024_s_199	9727071	( B)  Inhibition of CS-A binding  by PMA-treated K562  cells in the presence of  mAb Hermes-1 (8 mug/ml).	bind
167	2	851	6	NULL	NULL	0	NULL	Statement 1	NULL		occurs in presence of	NULL				mAb Hermes-1	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_102_5_1024_s_199	9727071	( B)  Inhibition of CS-A binding  by PMA-treated K562  cells in the presence of  mAb Hermes-1 (8 mug/ml).	bind
48238	1	851	7	NULL	NULL	0	NULL	K562 cells	Cells	PMA-treated	inhibit					 CS-A	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_5_1024_s_199	9727071	( B)  Inhibition of CS-A binding  by PMA-treated K562  cells in the presence of  mAb Hermes-1 (8 mug/ml).	bind
48239	2	851	7	NULL	NULL	0	NULL	statement 1	Process		in the presence of					mAb Hermes-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_5_1024_s_199	9727071	( B)  Inhibition of CS-A binding  by PMA-treated K562  cells in the presence of  mAb Hermes-1 (8 mug/ml).	bind
135	1	852	6	NULL	NULL	0	NULL	gp5/trx	NULL		bind	NULL				gp4E	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_14_5096_s_136	15795374	( B)  KD determination of the binding of gp5/trx to gp4E.	bind
48240	1	852	7	NULL	NULL	0	NULL	gp5/trx 	GP		bind					gp4E	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_14_5096_s_136	15795374	( B)  KD determination of the binding of gp5/trx to gp4E.	bind
136	1	853	6	10	NULL	0	NULL	Cdc42.GTPgammaS	NULL		bind	NULL					NULL		B-GBD		NULL		NULL	NULL	NULL	NULL	gw60_science_290_5492_801_s_105	11052943	( B)  PIP2 vesicle binding assays ( 29) show that  Cdc42.GTPgammaS and PIP2 can simultaneously bind the  control region (B-GBD).	bind
137	2	853	6	10	NULL	0	NULL	PIP2	NULL		bind	NULL					NULL		B-GBD		NULL		NULL	NULL	NULL	NULL	gw60_science_290_5492_801_s_105	11052943	( B)  PIP2 vesicle binding assays ( 29) show that  Cdc42.GTPgammaS and PIP2 can simultaneously bind the  control region (B-GBD).	bind
138	3	853	6	10	NULL	0	NULL	Statement 1	NULL		occur simultaneously with	NULL				Statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_science_290_5492_801_s_105	11052943	( B)  PIP2 vesicle binding assays ( 29) show that  Cdc42.GTPgammaS and PIP2 can simultaneously bind the  control region (B-GBD).	bind
50324	4	853	6	10	NULL	0	NULL	B-GBD	NULL		is a type of	NULL				control region	NULL				NULL		0	NULL	NULL	NULL	gw60_science_290_5492_801_s_105	11052943	( B)  PIP2 vesicle binding assays ( 29) show that  Cdc42.GTPgammaS and PIP2 can simultaneously bind the  control region (B-GBD).	bind
48241	1	853	7	NULL	NULL	0	NULL	Cdc42.GTPgammaS	GP		bind								B-GBD		NULL		NULL	NULL	NULL	NULL	gw60_science_290_5492_801_s_105	11052943	( B)  PIP2 vesicle binding assays ( 29) show that  Cdc42.GTPgammaS and PIP2 can simultaneously bind the  control region (B-GBD).	bind
48242	2	853	7	NULL	NULL	0	NULL	PIP2	GP		bind								B-GBD		NULL		NULL	NULL	NULL	NULL	gw60_science_290_5492_801_s_105	11052943	( B)  PIP2 vesicle binding assays ( 29) show that  Cdc42.GTPgammaS and PIP2 can simultaneously bind the  control region (B-GBD).	bind
48243	3	853	7	NULL	NULL	0	NULL	statement 1	Process		occur simultaneously with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_290_5492_801_s_105	11052943	( B)  PIP2 vesicle binding assays ( 29) show that  Cdc42.GTPgammaS and PIP2 can simultaneously bind the  control region (B-GBD).	bind
48244	4	853	7	NULL	NULL	0	NULL	B-GBD	GP		is a type of					control region	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_290_5492_801_s_105	11052943	( B)  PIP2 vesicle binding assays ( 29) show that  Cdc42.GTPgammaS and PIP2 can simultaneously bind the  control region (B-GBD).	bind
140	1	854	6	NULL	NULL	0	NULL	R-etodolac	NULL		bind	NULL	directly			RXRalpha	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_7_2525_s_146	15699354	( b)  R-etodolac binds directly to RXRalpha.	bind
48245	1	854	7	NULL	NULL	0	NULL	R-etodolac	Chemical		bind		directly			RXRalpha	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_7_2525_s_146	15699354	( b)  R-etodolac binds directly to RXRalpha.	bind
139	1	855	6	NULL	NULL	0	NULL	ZO-3	NULL		bind	NULL	directly			ZO-1	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_141_1_199_s_138	9531559	( b)  ZO-3 binds ZO-1 directly.	bind
48246	1	855	7	NULL	NULL	0	NULL	ZO-3 	GP		bind		directly			ZO-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_1_199_s_138	9531559	( b)  ZO-3 binds ZO-1 directly.	bind
141	1	856	6	10	NULL	0	NULL	gp120 IIIB	NULL	125I	bind	NULL				HeLa-CD4 cells	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_14_8005_s_133	9653130	( B) 125I-gp120 IIIB binding to HeLa-CD4 (clone H1-J) and to control HeLa cells.	bind
142	2	856	6	10	NULL	0	NULL	gp120 IIIB	NULL	125I	bind	NULL				HeLa cells	NULL	control			NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_14_8005_s_133	9653130	( B) 125I-gp120 IIIB binding to HeLa-CD4 (clone H1-J) and to control HeLa cells.	bind
48247	1	856	7	NULL	NULL	0	NULL	gp120 IIIB	GP	125I	bind					HeLa-CD4 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_14_8005_s_133	9653130	( B) 125I-gp120 IIIB binding to HeLa-CD4 (clone H1-J) and to control HeLa cells.	bind
48248	2	856	7	NULL	NULL	0	NULL	gp120 IIIB	GP	125I	bind					HeLa cells	Cell	control			NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_14_8005_s_133	9653130	( B) 125I-gp120 IIIB binding to HeLa-CD4 (clone H1-J) and to control HeLa cells.	bind
143	1	859	6	10	NULL	0	NULL	Sly1 	NULL	15N,13C-labeled	bind	NULL		N-terminal domain		syntaxin 5 peptide	NULL	unlabeled			NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_1_32_s_159	12506202	( B) 2D 13C-filtered, 13C-edited NOESY spectrum of 15N,13C-labeled Sly1 N-terminal domain bound to unlabeled syntaxin 5 peptide.	bind
48249	1	859	7	NULL	NULL	0	NULL	Sly1	GP	 15N,13C-labeled	bind			N-terminal domain		syntaxin 5 peptide	GP	unlabeled			NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_1_32_s_159	12506202	( B) 2D 13C-filtered, 13C-edited NOESY spectrum of 15N,13C-labeled Sly1 N-terminal domain bound to unlabeled syntaxin 5 peptide.	bind
144	1	861	6	NULL	NULL	0	NULL	40S pre-mRNP proteins	NULL		bind	NULL				DNase I 	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_8_1725_s_139	11937625	( B) 40S pre-mRNP proteins bound to DNase I - Sepharose and subsequently analyzed as in	bind
48250	1	861	7	NULL	NULL	0	NULL	40S pre-mRNP proteins	GP		bind					DNase I - Sepharose	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_8_1725_s_139	11937625	( B) 40S pre-mRNP proteins bound to DNase I - Sepharose and subsequently analyzed as in	bind
145	1	864	6	10	NULL	0	NULL	80R scFv	NULL		bind	NULL				S1-Ig	NULL		261 - 672		NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_8_2536_s_157	14983044	( B) 80R scFv bound to S1 (261 - 672)-Ig but did not bind to S1 (327)-Ig.	bind
146	2	864	6	10	NULL	0	NULL	80R scFv	NULL		does not bind	NULL				S1-Ig	NULL		327		NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_8_2536_s_157	14983044	( B) 80R scFv bound to S1 (261 - 672)-Ig but did not bind to S1 (327)-Ig.	bind
48251	1	864	7	NULL	NULL	0	NULL	 80R scFv	GP		bind					S1-Ig	GP		261 - 672		NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_8_2536_s_157	14983044	( B) 80R scFv bound to S1 (261 - 672)-Ig but did not bind to S1 (327)-Ig.	bind
48252	2	864	7	NULL	NULL	0	NULL	 80R scFv	GP		does not bind					S1-Ig	GP		327		NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_8_2536_s_157	14983044	( B) 80R scFv bound to S1 (261 - 672)-Ig but did not bind to S1 (327)-Ig.	bind
147	1	867	6	10	NULL	0	NULL	antibodies	NULL	tagged	bind	NULL				IgGs	NULL	chicken			NULL		NULL	NULL	NULL	NULL	gw60_science_276_5313_779_s_59	9115199	( B) A fluorescence micrograph shows light from tagged antibodies to chicken IgG that bound chicken IgGs patterned using a muFN as depicted in Fig.  1B.	bind
48253	1	867	7	NULL	NULL	0	NULL	antibodies	GP	tagged 	bind					IgG	GP	chicken			NULL		NULL	NULL	NULL	NULL	gw60_science_276_5313_779_s_59	9115199	( B) A fluorescence micrograph shows light from tagged antibodies to chicken IgG that bound chicken IgGs patterned using a muFN as depicted in Fig.  1B.	bind
148	1	868	6	NULL	NULL	0	NULL	clathrin	NULL		bind	NULL				GST - GGA2-hinge + GAE	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_22_1_78_s_173	12505986	( B) A mutant His6-Rabaptin-5 (5 - 476) fragment containing three alanine substitutions in codons 438 - 440 (5 - 476*) does not affect the binding of clathrin to GST - GGA2-hinge + GAE.	bind
149	2	868	6	10	NULL	0	NULL	His6-Rabaptin-5 fragment	NULL	mutant	contains	NULL				alanine substitutions	NULL		codons 438 - 440		NULL		NULL	NULL	NULL	NULL	gw60_embo_22_1_78_s_173	12505986	( B) A mutant His6-Rabaptin-5 (5 - 476) fragment containing three alanine substitutions in codons 438 - 440 (5 - 476*) does not affect the binding of clathrin to GST - GGA2-hinge + GAE.	bind
50325	3	868	6	10	NULL	0	NULL	Statement 2	NULL		does not affect	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_22_1_78_s_173	12505986	( B) A mutant His6-Rabaptin-5 (5 - 476) fragment containing three alanine substitutions in codons 438 - 440 (5 - 476*) does not affect the binding of clathrin to GST - GGA2-hinge + GAE.	bind
48254	1	868	7	NULL	NULL	0	NULL	clathrin	GP		bind					GST - GGA2-hinge + GAE	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_1_78_s_173	12505986	( B) A mutant His6-Rabaptin-5 (5 - 476) fragment containing three alanine substitutions in codons 438 - 440 (5 - 476*) does not affect the binding of clathrin to GST - GGA2-hinge + GAE.	bind
48255	2	868	7	NULL	NULL	0	NULL	His6-Rabaptin-5 fragment	GP	mutant	contains					alanine substitutions	AminoAcid		codons 438 - 440		NULL		NULL	NULL	NULL	NULL	gw60_embo_22_1_78_s_173	12505986	( B) A mutant His6-Rabaptin-5 (5 - 476) fragment containing three alanine substitutions in codons 438 - 440 (5 - 476*) does not affect the binding of clathrin to GST - GGA2-hinge + GAE.	bind
48256	3	868	7	NULL	NULL	0	NULL	statement 2	Process		does not affect					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_1_78_s_173	12505986	( B) A mutant His6-Rabaptin-5 (5 - 476) fragment containing three alanine substitutions in codons 438 - 440 (5 - 476*) does not affect the binding of clathrin to GST - GGA2-hinge + GAE.	bind
150	1	870	6	10	NULL	0	NULL	TNF ligands	NULL	Flag-tagged 	bind	NULL				BAFF-R:Fc	NULL				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5537_2108_s_70	11509692	( B) A panel of Flag-tagged TNF ligands was bound to BAFF-R:Fc, BCMA:Fc, or TACI:Fc coated plates and detected with the use of the HRP-M2 (Sigma).	bind
151	2	870	6	10	NULL	0	NULL	TNF ligands	NULL	Flag-tagged	bind	NULL				BCMA:Fc	NULL				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5537_2108_s_70	11509692	( B) A panel of Flag-tagged TNF ligands was bound to BAFF-R:Fc, BCMA:Fc, or TACI:Fc coated plates and detected with the use of the HRP-M2 (Sigma).	bind
152	3	870	6	10	NULL	0	NULL	TNF ligands	NULL	Flag-tagged	bind	NULL				TACI:Fc	NULL				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5537_2108_s_70	11509692	( B) A panel of Flag-tagged TNF ligands was bound to BAFF-R:Fc, BCMA:Fc, or TACI:Fc coated plates and detected with the use of the HRP-M2 (Sigma).	bind
48257	1	870	7	NULL	NULL	0	NULL	TNF ligands	GP	Flag-tagged	bind					 BAFF-R:Fc	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5537_2108_s_70	11509692	( B) A panel of Flag-tagged TNF ligands was bound to BAFF-R:Fc, BCMA:Fc, or TACI:Fc coated plates and detected with the use of the HRP-M2 (Sigma).	bind
48258	2	870	7	NULL	NULL	0	NULL	 TNF ligands	GP	Flag-tagged	bind					BCMA:Fc	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5537_2108_s_70	11509692	( B) A panel of Flag-tagged TNF ligands was bound to BAFF-R:Fc, BCMA:Fc, or TACI:Fc coated plates and detected with the use of the HRP-M2 (Sigma).	bind
48259	3	870	7	NULL	NULL	0	NULL	TNF ligands	GP	Flag-tagged	bind					TACI:Fc	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5537_2108_s_70	11509692	( B) A panel of Flag-tagged TNF ligands was bound to BAFF-R:Fc, BCMA:Fc, or TACI:Fc coated plates and detected with the use of the HRP-M2 (Sigma).	bind
153	1	872	6	NULL	NULL	0	NULL	Cdc11 septin	NULL		bind	NULL				Gin4	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_143_3_709_s_104	9813092	( B) A Western blot confirming that the Cdc11 septin binds to the Gin4 affinity column.	bind
48260	1	872	7	NULL	NULL	0	NULL	Cdc11 septin	GP		bind					Gin4	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_143_3_709_s_104	9813092	( B) A Western blot confirming that the Cdc11 septin binds to the Gin4 affinity column.	bind
154	1	874	6	10	NULL	0	NULL	Smad 3	NULL	activated	bind	NULL				c-jun probe	NULL	32P labeled			NULL	nuclear extracts	NULL	NULL	NULL	NULL	gw60_genesdev_14_20_2610_s_183	11040215	( B) Activated Smad3/4 binding to a 32P labeled c-jun probe was examined in nuclear extracts by EMSA.	bind
48261	1	874	7	NULL	NULL	0	NULL	Smad3/4	GP	activated	bind					c-jun probe	GP	32P labeled			NULL	nuclear extracts	NULL	NULL	NULL	NULL	gw60_genesdev_14_20_2610_s_183	11040215	( B) Activated Smad3/4 binding to a 32P labeled c-jun probe was examined in nuclear extracts by EMSA.	bind
155	1	875	6	NULL	NULL	0	NULL	PICK1	NULL		bind	NULL				GluR2	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_24_18_3266_s_317	16138078	( B) Activation of NMDARs localised in close proximity to AMPARs results in a Ca2+ flux that raises the local [Ca2+] to around 15 muM and therefore enhances binding of PICK1 to GluR2.	bind
156	2	875	6	NULL	NULL	0	NULL	NMDARs	NULL		localised in close proximity to	NULL				AMPARs	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_24_18_3266_s_317	16138078	( B) Activation of NMDARs localised in close proximity to AMPARs results in a Ca2+ flux that raises the local [Ca2+] to around 15 muM and therefore enhances binding of PICK1 to GluR2.	bind
157	3	875	6	NULL	NULL	0	NULL	NMDARs	NULL	activated	results in	NULL				Ca2+ flux	NULL				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_18_3266_s_317	16138078	( B) Activation of NMDARs localised in close proximity to AMPARs results in a Ca2+ flux that raises the local [Ca2+] to around 15 muM and therefore enhances binding of PICK1 to GluR2.	bind
158	4	875	6	NULL	NULL	0	NULL	Statement 3	NULL		enhances	NULL				Statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_24_18_3266_s_317	16138078	( B) Activation of NMDARs localised in close proximity to AMPARs results in a Ca2+ flux that raises the local [Ca2+] to around 15 muM and therefore enhances binding of PICK1 to GluR2.	bind
48262	1	875	7	NULL	NULL	0	NULL	NMDARs	GP		is in close proximity to					AMPARs	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_18_3266_s_317	16138078	( B) Activation of NMDARs localised in close proximity to AMPARs results in a Ca2+ flux that raises the local [Ca2+] to around 15 muM and therefore enhances binding of PICK1 to GluR2.	bind
48263	2	875	7	NULL	NULL	0	NULL	statement 1	Process	activation of	result in					Ca2+ flux	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_18_3266_s_317	16138078	( B) Activation of NMDARs localised in close proximity to AMPARs results in a Ca2+ flux that raises the local [Ca2+] to around 15 muM and therefore enhances binding of PICK1 to GluR2.	bind
48264	3	875	7	NULL	NULL	0	NULL	statement 2	Process		leads to					Ca2+	Chemical	increase in			NULL		NULL	NULL	NULL	NULL	gw70_embo_24_18_3266_s_317	16138078	( B) Activation of NMDARs localised in close proximity to AMPARs results in a Ca2+ flux that raises the local [Ca2+] to around 15 muM and therefore enhances binding of PICK1 to GluR2.	bind
48265	4	875	7	NULL	NULL	0	NULL	PICK1	GP		bind					GluR2	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_18_3266_s_317	16138078	( B) Activation of NMDARs localised in close proximity to AMPARs results in a Ca2+ flux that raises the local [Ca2+] to around 15 muM and therefore enhances binding of PICK1 to GluR2.	bind
48266	5	875	7	NULL	NULL	0	NULL	statement 3	Process		enhance					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_18_3266_s_317	16138078	( B) Activation of NMDARs localised in close proximity to AMPARs results in a Ca2+ flux that raises the local [Ca2+] to around 15 muM and therefore enhances binding of PICK1 to GluR2.	bind
159	1	876	6	NULL	NULL	0	NULL	CN5	NULL		bind	NULL				F-actin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_5_3089_s_243	12446728	( B) addition of TnI to the Tm.TnT binary complex slightly increased the inhibitory effect  on CN5 binding to F-actin.	bind
160	2	876	6	10	NULL	0	NULL	TnI	NULL		added to	NULL				Tm.TnT binary complex	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_5_3089_s_243	12446728	( B) addition of TnI to the Tm.TnT binary complex slightly increased the inhibitory effect  on CN5 binding to F-actin.	bind
161	3	876	6	10	NULL	0	NULL	Statement 2	NULL		increases	NULL				statement 1                                                                                                                                                                                                                                                  	NULL	inhibitory effect of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_5_3089_s_243	12446728	( B) addition of TnI to the Tm.TnT binary complex slightly increased the inhibitory effect  on CN5 binding to F-actin.	bind
48267	1	876	7	NULL	NULL	0	NULL	CN5	GP		bind					F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_5_3089_s_243	12446728	( B) addition of TnI to the Tm.TnT binary complex slightly increased the inhibitory effect  on CN5 binding to F-actin.	bind
48268	2	876	7	NULL	NULL	0	NULL	TnI	GP		added to					Tm.TnT binary complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_5_3089_s_243	12446728	( B) addition of TnI to the Tm.TnT binary complex slightly increased the inhibitory effect  on CN5 binding to F-actin.	bind
48269	3	876	7	NULL	NULL	0	NULL	statement 2	Process		increase					statement 1	Process	inhibitory effect of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_5_3089_s_243	12446728	( B) addition of TnI to the Tm.TnT binary complex slightly increased the inhibitory effect  on CN5 binding to F-actin.	bind
162	1	878	6	NULL	NULL	0	NULL	ADP	NULL		bind	NULL				GroEL	NULL				NULL		0	NULL	NULL	NULL	gw60_annrevbiochem_67_0_581_s_207	9759498	( B) ADP bound to GroEL in the   GroEL-GroES-(ADP)7 structure.	bind
48270	1	878	7	NULL	NULL	0	NULL	ADP	Chemical		bind					 GroEL	GP				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_67_0_581_s_207	9759498	( B) ADP bound to GroEL in the   GroEL-GroES-(ADP)7 structure.	bind
164	1	880	6	NULL	NULL	0	NULL	Six3	NULL		bind	NULL				Crygf	NULL			promoter sequences	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_2_515_s_238	11139622	( b) Affinity binding of Six3 to  Crygf promoter sequences.	bind
48272	1	880	7	NULL	NULL	0	NULL	 Six3	GP		bind					 Crygf	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_2_515_s_238	11139622	( b) Affinity binding of Six3 to  Crygf promoter sequences.	bind
163	1	882	6	NULL	NULL	0	NULL	IP3	NULL		bind	NULL				IP3R	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_437_s_220	15189149	( B) After agonist stimulus, IP3 binds to the IP3R, causing a conformational change in the channel.	bind
50326	2	882	6	10	NULL	0	NULL	statement 1	NULL		occurs after	NULL				agonist	NULL	stimulus of			NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_437_s_220	15189149	( B) After agonist stimulus, IP3 binds to the IP3R, causing a conformational change in the channel.	bind
50327	3	882	6	10	NULL	0	NULL	statement 1	NULL		causes	NULL				channel	NULL	conformational change of			NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_437_s_220	15189149	( B) After agonist stimulus, IP3 binds to the IP3R, causing a conformational change in the channel.	bind
48273	1	882	7	NULL	NULL	0	NULL	IP3	Chemical		bind					IP3R	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_73_0_437_s_220	15189149	( B) After agonist stimulus, IP3 binds to the IP3R, causing a conformational change in the channel.	bind
48274	2	882	7	NULL	NULL	0	NULL	statement 1	Process		occurs after					agonist	Chemical	stimulus by			NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_73_0_437_s_220	15189149	( B) After agonist stimulus, IP3 binds to the IP3R, causing a conformational change in the channel.	bind
48275	3	882	7	NULL	NULL	0	NULL	statement 1	Process		cause					channel	CellComponent	conformational change of			NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_73_0_437_s_220	15189149	( B) After agonist stimulus, IP3 binds to the IP3R, causing a conformational change in the channel.	bind
174	1	883	6	NULL	NULL	0	NULL	GroES	NULL		bind	NULL				GroEL	NULL		First ring		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_52_32925_s_27	9407071	( b) After GroES binding to one GroEL ring to form an asymmetric complex, the second ring seems to bind a second GroES molecule to form a symmetric complex with lower affinity ( 14).	bind
175	2	883	6	NULL	NULL	0	NULL	Statement 1	NULL		forms an	NULL				asymmetric complex	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_52_32925_s_27	9407071	( b) After GroES binding to one GroEL ring to form an asymmetric complex, the second ring seems to bind a second GroES molecule to form a symmetric complex with lower affinity ( 14).	bind
176	3	883	6	NULL	NULL	0	NULL	GroES	NULL		bind	NULL				GroEL 	NULL		second ring		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_52_32925_s_27	9407071	( b) After GroES binding to one GroEL ring to form an asymmetric complex, the second ring seems to bind a second GroES molecule to form a symmetric complex with lower affinity ( 14).	bind
177	4	883	6	NULL	NULL	0	NULL	Statement 3	NULL		forms a	NULL				symmetric complex	NULL	lower affinity			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_52_32925_s_27	9407071	( b) After GroES binding to one GroEL ring to form an asymmetric complex, the second ring seems to bind a second GroES molecule to form a symmetric complex with lower affinity ( 14).	bind
50329	5	883	6	10	NULL	0	NULL	statement 3	NULL		occurs after	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_52_32925_s_27	9407071	( b) After GroES binding to one GroEL ring to form an asymmetric complex, the second ring seems to bind a second GroES molecule to form a symmetric complex with lower affinity ( 14).	bind
48276	1	883	7	NULL	NULL	0	NULL	GroES	GP		bind					GroEL 	GP		first ring		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_52_32925_s_27	9407071	( b) After GroES binding to one GroEL ring to form an asymmetric complex, the second ring seems to bind a second GroES molecule to form a symmetric complex with lower affinity ( 14).	bind
48277	2	883	7	NULL	NULL	0	NULL	statement 1	Process		forms					asymmetric complex					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_52_32925_s_27	9407071	( b) After GroES binding to one GroEL ring to form an asymmetric complex, the second ring seems to bind a second GroES molecule to form a symmetric complex with lower affinity ( 14).	bind
48278	3	883	7	NULL	NULL	0	NULL	GroES	GP		bind					GroEL	GP		second ring		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_52_32925_s_27	9407071	( b) After GroES binding to one GroEL ring to form an asymmetric complex, the second ring seems to bind a second GroES molecule to form a symmetric complex with lower affinity ( 14).	bind
48279	4	883	7	NULL	NULL	0	NULL	statement 3	Process		forms		low affinity			symmetric complex					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_52_32925_s_27	9407071	( b) After GroES binding to one GroEL ring to form an asymmetric complex, the second ring seems to bind a second GroES molecule to form a symmetric complex with lower affinity ( 14).	bind
48280	5	883	7	NULL	NULL	0	NULL	statement 3	Process		occurs after					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_52_32925_s_27	9407071	( b) After GroES binding to one GroEL ring to form an asymmetric complex, the second ring seems to bind a second GroES molecule to form a symmetric complex with lower affinity ( 14).	bind
165	1	887	6	10	NULL	0	NULL	DEBP	NULL		bind	NULL				goosecoid DE	NULL				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_4_435_s_54	10691736	( B) An activin-inducible protein (DEBP) binds the  goosecoid DE.	bind
50330	2	887	6	10	NULL	0	NULL	DEBP	NULL		is a type of	NULL				activin-inducible protein	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_14_4_435_s_54	10691736	( B) An activin-inducible protein (DEBP) binds the  goosecoid DE.	bind
48281	1	887	7	NULL	NULL	0	NULL	DEBP	GP		bind					 goosecoid 	GP			DE	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_4_435_s_54	10691736	( B) An activin-inducible protein (DEBP) binds the  goosecoid DE.	bind
48282	2	887	7	NULL	NULL	0	NULL	DEBP	GP		is a type of					activin-inducible protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_4_435_s_54	10691736	( B) An activin-inducible protein (DEBP) binds the  goosecoid DE.	bind
178	1	888	6	10	NULL	0	NULL	p53	NULL	bacterially purified	bind	NULL	sequence-specific 			XPC-p53	NULL			 response element	NULL	In vitro	NULL	NULL	NULL	NULL	gw60_pnas_99_20_12985_s_163	12242345	( B) An electrophoretic mobility-shift assay demonstrates sequence-specific DNA binding of bacterially purified p53 to the identified  XPC-p53 response element  in vitro.	bind
48283	1	888	7	NULL	NULL	0	NULL	p53	GP	bacterially purified	bind		sequence-specific			XPC-p53 	GP			response element	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_pnas_99_20_12985_s_163	12242345	( B) An electrophoretic mobility-shift assay demonstrates sequence-specific DNA binding of bacterially purified p53 to the identified  XPC-p53 response element  in vitro.	bind
179	1	889	6	10	NULL	0	NULL	C3d mAb	NULL	Alexa Fluor 647 labelled	bind	NULL				IAM	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_115_5_1241_s_140	15849610	( B) An mAb to C3d labeled with Alexa Fluor 647 binds to the IAM.	bind
48284	1	889	7	NULL	NULL	0	NULL	 C3d mAb	GP	 Alexa Fluor 647 labeled	bind					IAM	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_115_5_1241_s_140	15849610	( B) An mAb to C3d labeled with Alexa Fluor 647 binds to the IAM.	bind
180	1	891	6	NULL	NULL	0	NULL	MxiD	NULL		bind	NULL				MxiM	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_24_6_1111_s_176	15775974	( B) Analysis of MxiD binding to MxiM incubated with the lipid 2-dioctanoylsnnglycero-3-phosphate.	bind
48286	1	891	7	NULL	NULL	0	NULL	MxiD 	GP		bind					MxiM	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_6_1111_s_176	15775974	( B) Analysis of MxiD binding to MxiM incubated with the lipid 2-dioctanoylsnnglycero-3-phosphate.	bind
181	1	892	6	NULL	NULL	0	NULL	Nap1p	NULL		binds to	NULL				GST - histone	NULL		N-terminal tails		NULL		0	NULL	NULL	NULL	gw60_embo_21_23_6527_s_101	12456659	( B) Analysis of Nap1p binding to GST - histone N-terminal tails (1 muM of each) as in	bind
48287	1	892	7	NULL	NULL	0	NULL	Nap1p	GP		bind					 GST - histone	GP		N-terminal tails		NULL		NULL	NULL	NULL	NULL	gw60_embo_21_23_6527_s_101	12456659	( B) Analysis of Nap1p binding to GST - histone N-terminal tails (1 muM of each) as in	bind
182	1	894	6	NULL	NULL	0	NULL	Sp1	NULL		bind	NULL				DNA	NULL			GC box	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_15_4523_s_134	12888513	( B) Analysis of the effect of pH and ZnCl2 on Sp1 binding to GC box DNA in the DNA binding assay.	bind
48288	1	894	7	NULL	NULL	0	NULL	Sp1	GP		bind					DNA	NucleicAcid			GC box	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_15_4523_s_134	12888513	( B) Analysis of the effect of pH and ZnCl2 on Sp1 binding to GC box DNA in the DNA binding assay.	bind
183	1	895	6	NULL	NULL	0	NULL	UL28 protein	NULL		bind	NULL				Ub DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_98_6_3086_s_112	11248036	( B) Analysis of UL28 protein binding to Ub DNA.	bind
48289	1	895	7	NULL	NULL	0	NULL	UL28 protein	GP		bind					Ub DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_6_3086_s_112	11248036	( B) Analysis of UL28 protein binding to Ub DNA.	bind
185	1	896	6	10	NULL	0	NULL	NIP1-N	NULL		binds to	NULL				eIF1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_19_2534_s_57	11018020	( B) and ( C) The amino-terminal segment of eIF3-NIP1 (NIP1-N) binds to eIF1 and eIF5.	bind
186	2	896	6	10	NULL	0	NULL	NIP1-N	NULL		bind	NULL				eIF5	NULL				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_19_2534_s_57	11018020	( B) and ( C) The amino-terminal segment of eIF3-NIP1 (NIP1-N) binds to eIF1 and eIF5.	bind
50331	3	896	6	10	NULL	0	NULL	NIP1-N	NULL		is	NULL				amino-terminal segment of eIF3-NIP1	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_14_19_2534_s_57	11018020	( B) and ( C) The amino-terminal segment of eIF3-NIP1 (NIP1-N) binds to eIF1 and eIF5.	bind
48290	1	896	7	NULL	NULL	0	NULL	NIP1-N	GP		bind					eIF1	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_19_2534_s_57	11018020	( B) and ( C) The amino-terminal segment of eIF3-NIP1 (NIP1-N) binds to eIF1 and eIF5.	bind
48291	2	896	7	NULL	NULL	0	NULL	NIP1-N	GP		bind					eIF5	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_19_2534_s_57	11018020	( B) and ( C) The amino-terminal segment of eIF3-NIP1 (NIP1-N) binds to eIF1 and eIF5.	bind
48292	3	896	7	NULL	NULL	0	NULL	NIP1-N	GP		is					amino-terminal segment of eIF3-NIP1	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_19_2534_s_57	11018020	( B) and ( C) The amino-terminal segment of eIF3-NIP1 (NIP1-N) binds to eIF1 and eIF5.	bind
187	1	897	6	NULL	NULL	0	NULL	LGL	NULL	leukemic	bind	NULL				PBMCs	NULL	normal			NULL		0	NULL	NULL	NULL	gw60_jclininvest_107_3_351_s_147	11160159	( b) Annexin-V-FITC binding of leukemic LGL and normal PBMCs in response to DMSO (0) and AG-490 (25, 50, and 100 muM for 48 hours).	bind
48293	1	897	7	NULL	NULL	0	NULL	 Annexin-V-FITC	GP		bind					leukemic LGL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_107_3_351_s_147	11160159	( b) Annexin-V-FITC binding of leukemic LGL and normal PBMCs in response to DMSO (0) and AG-490 (25, 50, and 100 muM for 48 hours).	bind
48294	2	897	7	NULL	NULL	0	NULL	Annexin-V-FITC	GP		bind					PBMCs	Cell	normal			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_107_3_351_s_147	11160159	( b) Annexin-V-FITC binding of leukemic LGL and normal PBMCs in response to DMSO (0) and AG-490 (25, 50, and 100 muM for 48 hours).	bind
48295	3	897	7	NULL	NULL	0	NULL	statement 1	Process		in response to					DMSO	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_107_3_351_s_147	11160159	( b) Annexin-V-FITC binding of leukemic LGL and normal PBMCs in response to DMSO (0) and AG-490 (25, 50, and 100 muM for 48 hours).	bind
48296	4	897	7	NULL	NULL	0	NULL	statement 1	Process		in response to					AG-490	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_107_3_351_s_147	11160159	( b) Annexin-V-FITC binding of leukemic LGL and normal PBMCs in response to DMSO (0) and AG-490 (25, 50, and 100 muM for 48 hours).	bind
48297	5	897	7	NULL	NULL	0	NULL	statement 2	Process		in response to					DMSO	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_107_3_351_s_147	11160159	( b) Annexin-V-FITC binding of leukemic LGL and normal PBMCs in response to DMSO (0) and AG-490 (25, 50, and 100 muM for 48 hours).	bind
48298	6	897	7	NULL	NULL	0	NULL	statement 2	Process		in response to					AG-490	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_107_3_351_s_147	11160159	( b) Annexin-V-FITC binding of leukemic LGL and normal PBMCs in response to DMSO (0) and AG-490 (25, 50, and 100 muM for 48 hours).	bind
188	1	899	6	10	NULL	0	NULL	p65	NULL		bind	NULL				NF-kappaB	NULL			response element	NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_1_43_s_223	16000401	( B) Antibodies against p65, p50 and c-Rel supershift the nuclear protein binding to  the NF-kappaB response elements.	bind
189	2	899	6	10	NULL	0	NULL	p50	NULL		bind	NULL				NF-kappaB	NULL			response element	NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_1_43_s_223	16000401	( B) Antibodies against p65, p50 and c-Rel supershift the nuclear protein binding to  the NF-kappaB response elements.	bind
190	3	899	6	10	NULL	0	NULL	c-Rel	NULL		bind	NULL				NF-kappaB	NULL			response element	NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_1_43_s_223	16000401	( B) Antibodies against p65, p50 and c-Rel supershift the nuclear protein binding to  the NF-kappaB response elements.	bind
51429	4	899	6	10	NULL	0	NULL	p65	NULL		is a type of	NULL				nuclear protein	NULL				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_27_1_43_s_223	16000401	( B) Antibodies against p65, p50 and c-Rel supershift the nuclear protein binding to  the NF-kappaB response elements.	bind
51430	5	899	6	10	NULL	0	NULL	p50	NULL		is a type of	NULL				nuclear protein	NULL				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_27_1_43_s_223	16000401	( B) Antibodies against p65, p50 and c-Rel supershift the nuclear protein binding to  the NF-kappaB response elements.	bind
51431	6	899	6	10	NULL	0	NULL	c-Rel	NULL		is a type of	NULL				nuclear protein	NULL				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_27_1_43_s_223	16000401	( B) Antibodies against p65, p50 and c-Rel supershift the nuclear protein binding to  the NF-kappaB response elements.	bind
48299	1	899	7	NULL	NULL	0	NULL	 p65	GP		bind					NF-kappaB	GP			response element	NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_1_43_s_223	16000401	( B) Antibodies against p65, p50 and c-Rel supershift the nuclear protein binding to  the NF-kappaB response elements.	bind
48300	2	899	7	NULL	NULL	0	NULL	p50	GP		bind					NF-kappaB	GP			response element	NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_1_43_s_223	16000401	( B) Antibodies against p65, p50 and c-Rel supershift the nuclear protein binding to  the NF-kappaB response elements.	bind
48301	3	899	7	NULL	NULL	0	NULL	c-Rel	GP		bind					NF-kappaB	GP			response element	NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_1_43_s_223	16000401	( B) Antibodies against p65, p50 and c-Rel supershift the nuclear protein binding to  the NF-kappaB response elements.	bind
48302	4	899	7	NULL	NULL	0	NULL	p65	GP		is a type of					nuclear protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_1_43_s_223	16000401	( B) Antibodies against p65, p50 and c-Rel supershift the nuclear protein binding to  the NF-kappaB response elements.	bind
48303	5	899	7	NULL	NULL	0	NULL	p50	GP		is a type of					nuclear protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_1_43_s_223	16000401	( B) Antibodies against p65, p50 and c-Rel supershift the nuclear protein binding to  the NF-kappaB response elements.	bind
48304	6	899	7	NULL	NULL	0	NULL	c-Rel	GP		is a type of					nuclear protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_1_43_s_223	16000401	( B) Antibodies against p65, p50 and c-Rel supershift the nuclear protein binding to  the NF-kappaB response elements.	bind
191	1	900	6	10	NULL	0	NULL	SIVmac239 gp120	NULL	125I-labeled	binds to	NULL				CCR5	NULL	rhesus			NULL		NULL	NULL	NULL	NULL	gw60_science_278_5342_1470_s_69	9367961	( B) Antibody inhibition of 125I-labeled SIVmac239 gp120 binding to rhesus CCR5 in the presence (solid bars) or absence (open bars) of 100 nM sCD4.	bind
48305	1	900	7	NULL	NULL	0	NULL	SIVmac239 gp120	GP	125I-labeled 	bind					CCR5	GP	rhesus			NULL		NULL	NULL	NULL	NULL	gw60_science_278_5342_1470_s_69	9367961	( B) Antibody inhibition of 125I-labeled SIVmac239 gp120 binding to rhesus CCR5 in the presence (solid bars) or absence (open bars) of 100 nM sCD4.	bind
193	1	903	6	10	NULL	0	NULL	regulatory proteins	NULL		bind	NULL		ChrD		Lys-9	NULL	methylated			NULL		NULL	NULL	NULL	NULL	gw60_science_292_5514_64_s_46	11294220	( B) As a result of these modifications, the chromodomain (ChrD) of regulatory proteins binds to methylated Lys-9 during gene silencing, and the bromodomain (BrD) of regulatory proteins binds to acetylated Lys-14 during gene activation.	bind
194	2	903	6	NULL	NULL	0	NULL	Statement 1	NULL		occurs during	NULL				gene silencing	NULL				NULL		0	NULL	NULL	NULL	gw60_science_292_5514_64_s_46	11294220	( B) As a result of these modifications, the chromodomain (ChrD) of regulatory proteins binds to methylated Lys-9 during gene silencing, and the bromodomain (BrD) of regulatory proteins binds to acetylated Lys-14 during gene activation.	bind
195	3	903	6	10	NULL	0	NULL	regulatory proteins	NULL		bind	NULL		BrD		Lys-14	NULL	acetylated			NULL		NULL	NULL	NULL	NULL	gw60_science_292_5514_64_s_46	11294220	( B) As a result of these modifications, the chromodomain (ChrD) of regulatory proteins binds to methylated Lys-9 during gene silencing, and the bromodomain (BrD) of regulatory proteins binds to acetylated Lys-14 during gene activation.	bind
196	4	903	6	NULL	NULL	0	NULL	Statement 3	NULL		occurs during	NULL				gene activation	NULL				NULL		0	NULL	NULL	NULL	gw60_science_292_5514_64_s_46	11294220	( B) As a result of these modifications, the chromodomain (ChrD) of regulatory proteins binds to methylated Lys-9 during gene silencing, and the bromodomain (BrD) of regulatory proteins binds to acetylated Lys-14 during gene activation.	bind
51432	5	903	6	10	NULL	0	NULL	ChrD	NULL		is	NULL				chromodomain	NULL				NULL		0	NULL	NULL	NULL	gw60_science_292_5514_64_s_46	11294220	( B) As a result of these modifications, the chromodomain (ChrD) of regulatory proteins binds to methylated Lys-9 during gene silencing, and the bromodomain (BrD) of regulatory proteins binds to acetylated Lys-14 during gene activation.	bind
51433	6	903	6	10	NULL	0	NULL	BrD	NULL		is	NULL				bromodomain	NULL				NULL		0	NULL	NULL	NULL	gw60_science_292_5514_64_s_46	11294220	( B) As a result of these modifications, the chromodomain (ChrD) of regulatory proteins binds to methylated Lys-9 during gene silencing, and the bromodomain (BrD) of regulatory proteins binds to acetylated Lys-14 during gene activation.	bind
48306	1	903	7	NULL	NULL	0	NULL	regulatory protein	GP		bind			ChrD				methylated	Lys-9		NULL		NULL	NULL	NULL	NULL	gw60_science_292_5514_64_s_46	11294220	( B) As a result of these modifications, the chromodomain (ChrD) of regulatory proteins binds to methylated Lys-9 during gene silencing, and the bromodomain (BrD) of regulatory proteins binds to acetylated Lys-14 during gene activation.	bind
48307	2	903	7	NULL	NULL	0	NULL	statement 1	Process		occurs during					gene silencing	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_292_5514_64_s_46	11294220	( B) As a result of these modifications, the chromodomain (ChrD) of regulatory proteins binds to methylated Lys-9 during gene silencing, and the bromodomain (BrD) of regulatory proteins binds to acetylated Lys-14 during gene activation.	bind
48308	3	903	7	NULL	NULL	0	NULL	regulatory protein	GP		bind			BrD				acetylated	Lys-14		NULL		NULL	NULL	NULL	NULL	gw60_science_292_5514_64_s_46	11294220	( B) As a result of these modifications, the chromodomain (ChrD) of regulatory proteins binds to methylated Lys-9 during gene silencing, and the bromodomain (BrD) of regulatory proteins binds to acetylated Lys-14 during gene activation.	bind
48309	4	903	7	NULL	NULL	0	NULL	statement 3	Process		occurs during					gene activation	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_292_5514_64_s_46	11294220	( B) As a result of these modifications, the chromodomain (ChrD) of regulatory proteins binds to methylated Lys-9 during gene silencing, and the bromodomain (BrD) of regulatory proteins binds to acetylated Lys-14 during gene activation.	bind
48310	5	903	7	NULL	NULL	0	NULL				is			ChrD		chromodomain	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_292_5514_64_s_46	11294220	( B) As a result of these modifications, the chromodomain (ChrD) of regulatory proteins binds to methylated Lys-9 during gene silencing, and the bromodomain (BrD) of regulatory proteins binds to acetylated Lys-14 during gene activation.	bind
48311	6	903	7	NULL	NULL	0	NULL				is			BrD		Bromodomain	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_292_5514_64_s_46	11294220	( B) As a result of these modifications, the chromodomain (ChrD) of regulatory proteins binds to methylated Lys-9 during gene silencing, and the bromodomain (BrD) of regulatory proteins binds to acetylated Lys-14 during gene activation.	bind
197	1	904	6	NULL	NULL	0	NULL	calpain	NULL		cleave	NULL				BM-V	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_29_17561_s_191	8663447	( b) Assessment of the actin binding properties of the calpain cleavage products of BM-V indicates that the 80-kDa tail fragment does not bind F-actin.	bind
198	2	904	6	10	NULL	0	NULL	BM-V	NULL		does not bind	NULL		80-kDa tail fragment		F-actin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_29_17561_s_191	8663447	( b) Assessment of the actin binding properties of the calpain cleavage products of BM-V indicates that the 80-kDa tail fragment does not bind F-actin.	bind
48312	1	904	7	NULL	NULL	0	NULL	BM-V	GP		does not bind			80-kDa tail fragment		F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_29_17561_s_191	8663447	( b) Assessment of the actin binding properties of the calpain cleavage products of BM-V indicates that the 80-kDa tail fragment does not bind F-actin.	bind
48313	2	904	7	NULL	NULL	0	NULL	calpain	GP		cleaves					BM-V	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_29_17561_s_191	8663447	( b) Assessment of the actin binding properties of the calpain cleavage products of BM-V indicates that the 80-kDa tail fragment does not bind F-actin.	bind
199	1	905	6	NULL	NULL	0	NULL	U1C	NULL		bind	NULL				ps5	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_101_41_14841_s_181	15465910	( B) At higher temperatures (indicated by kt), there is a conformational change (indicated  by a double arrow in  A) that includes U1C binding to the ps5''.	bind
48314	1	905	7	NULL	NULL	0	NULL	U1C	GP		bind					ps5''	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_41_14841_s_181	15465910	( B) At higher temperatures (indicated by kt), there is a conformational change (indicated  by a double arrow in  A) that includes U1C binding to the ps5''.	bind
200	1	906	6	10	NULL	0	NULL	p53c	NULL		bind	NULL				HIF-1alpha peptide	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_16_10305_s_31	12124396	( b) Average of three immunoblot experiments of p53c bound to HIF-1alpha peptide array.	bind
48315	1	906	7	NULL	NULL	0	NULL	p53c	GP		bind					 HIF-1alpha peptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_16_10305_s_31	12124396	( b) Average of three immunoblot experiments of p53c bound to HIF-1alpha peptide array.	bind
201	1	907	6	NULL	NULL	0	NULL	QK	NULL		bind	NULL				Flt-1D2	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_40_14215_s_122	16186493	( b) Backbone superposition of the QK representative structure (yellow) and VEGF helix  (red) bound to Flt-1D2.	bind
202	2	907	6	NULL	NULL	0	NULL	VEGF helix	NULL		bind	NULL				Flt-1D2	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_40_14215_s_122	16186493	( b) Backbone superposition of the QK representative structure (yellow) and VEGF helix  (red) bound to Flt-1D2.	bind
48316	1	907	7	NULL	NULL	0	NULL	VEGF helix	GP		bind					Flt-1D2	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_40_14215_s_122	16186493	( b) Backbone superposition of the QK representative structure (yellow) and VEGF helix  (red) bound to Flt-1D2.	bind
51434	2	907	7	NULL	NULL	0	NULL	QK	GP		bind					Flt-1D2	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_40_14215_s_122	16186493	( b) Backbone superposition of the QK representative structure (yellow) and VEGF helix  (red) bound to Flt-1D2.	bind
204	1	911	6	10	NULL	0	NULL	BMP-2 variants	NULL		bind	NULL				BMPR-II	NULL				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_13_3314_s_121	10880444	( B) Binding affinity of BMP-2 variants for type II receptors BMPR-II or ActR-II.	bind
205	2	911	6	10	NULL	0	NULL	BMP-2 variants	NULL		bind	NULL				ActR-II	NULL				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_13_3314_s_121	10880444	( B) Binding affinity of BMP-2 variants for type II receptors BMPR-II or ActR-II.	bind
51435	3	911	6	10	NULL	0	NULL	BMPR-II	NULL		is a type of	NULL				type II receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_19_13_3314_s_121	10880444	( B) Binding affinity of BMP-2 variants for type II receptors BMPR-II or ActR-II.	bind
51436	4	911	6	10	NULL	0	NULL	ActR-II	NULL		is a type of	NULL				type II receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_19_13_3314_s_121	10880444	( B) Binding affinity of BMP-2 variants for type II receptors BMPR-II or ActR-II.	bind
48317	1	911	7	NULL	NULL	0	NULL	BMP-2 variants	GP		bind					BMPR-II	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_13_3314_s_121	10880444	( B) Binding affinity of BMP-2 variants for type II receptors BMPR-II or ActR-II.	bind
48318	2	911	7	NULL	NULL	0	NULL	BMP-2 variants	GP		bind					ActR-II	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_13_3314_s_121	10880444	( B) Binding affinity of BMP-2 variants for type II receptors BMPR-II or ActR-II.	bind
48319	3	911	7	NULL	NULL	0	NULL	BMPR-II	GP		is a type of					type II receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_13_3314_s_121	10880444	( B) Binding affinity of BMP-2 variants for type II receptors BMPR-II or ActR-II.	bind
48320	4	911	7	NULL	NULL	0	NULL	ActR-II	GP		is a type of					type II receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_13_3314_s_121	10880444	( B) Binding affinity of BMP-2 variants for type II receptors BMPR-II or ActR-II.	bind
206	1	912	6	NULL	NULL	0	NULL	Cry11Aa	NULL		bind	NULL				Cyt1Aa	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_51_18303_s_112	16339907	( B) Binding analysis of Cry11Aa or Cry1Ab to Cyt1Aa by ELISA.	bind
207	2	912	6	NULL	NULL	0	NULL	Cry1Ab	NULL		bind	NULL				Cyt1Aa	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_51_18303_s_112	16339907	( B) Binding analysis of Cry11Aa or Cry1Ab to Cyt1Aa by ELISA.	bind
51437	3	912	6	10	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_51_18303_s_112	16339907	( B) Binding analysis of Cry11Aa or Cry1Ab to Cyt1Aa by ELISA.	bind
48321	1	912	7	NULL	NULL	0	NULL	Cry11Aa	GP		bind					Cyt1Aa	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_51_18303_s_112	16339907	( B) Binding analysis of Cry11Aa or Cry1Ab to Cyt1Aa by ELISA.	bind
48322	2	912	7	NULL	NULL	0	NULL	Cry1Ab	GP		bind					Cyt1Aa	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_51_18303_s_112	16339907	( B) Binding analysis of Cry11Aa or Cry1Ab to Cyt1Aa by ELISA.	bind
48323	3	912	7	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_51_18303_s_112	16339907	( B) Binding analysis of Cry11Aa or Cry1Ab to Cyt1Aa by ELISA.	bind
213	1	913	6	10	NULL	0	NULL	Chk1	NULL		bind	NULL				Pds1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5442_1166_s_90	10550056	( B) Binding and phosphorylation of Pds1 by Chk1.	bind
214	2	913	6	10	NULL	0	NULL	statement 1	NULL		phosphorylates	NULL				Pds1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5442_1166_s_90	10550056	( B) Binding and phosphorylation of Pds1 by Chk1.	bind
48324	1	913	7	NULL	NULL	0	NULL	Chk1	GP		bind					Pds1	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5442_1166_s_90	10550056	( B) Binding and phosphorylation of Pds1 by Chk1.	bind
48325	2	913	7	NULL	NULL	0	NULL	statement 1	Process		phosphorylate					Pds1	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5442_1166_s_90	10550056	( B) Binding and phosphorylation of Pds1 by Chk1.	bind
215	1	914	6	10	NULL	0	NULL	S1	NULL	His6-tagged	bind	NULL				PK1L SsrA variant	NULL	32P-labeled			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_6_3040_s_132	11248028	( B) Binding curve generated from data in  A. ( C) Binding of His6-tagged ribosomal protein S1 to 100 pM 32P-labeled PK1L and PK3L SsrA variants.	bind
216	2	914	6	10	NULL	0	NULL	S1	NULL	His6-tagged	bind	NULL				PK3L SsrA variant	NULL	32P-labeled			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_6_3040_s_132	11248028	( B) Binding curve generated from data in  A. ( C) Binding of His6-tagged ribosomal protein S1 to 100 pM 32P-labeled PK1L and PK3L SsrA variants.	bind
51438	3	914	6	10	NULL	0	NULL	S1	NULL		is a type of	NULL				ribosomal protein	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_98_6_3040_s_132	11248028	( B) Binding curve generated from data in  A. ( C) Binding of His6-tagged ribosomal protein S1 to 100 pM 32P-labeled PK1L and PK3L SsrA variants.	bind
48326	1	914	7	NULL	NULL	0	NULL	S1 	GP	His6-tagged	bind					PK1L SsrA variant	GP	32P-labeled			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_6_3040_s_132	11248028	( B) Binding curve generated from data in  A. ( C) Binding of His6-tagged ribosomal protein S1 to 100 pM 32P-labeled PK1L and PK3L SsrA variants.	bind
48327	2	914	7	NULL	NULL	0	NULL	S1	GP	His6-tagged 	bind					PK3L SsrA variant	GP	32P-labeled			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_6_3040_s_132	11248028	( B) Binding curve generated from data in  A. ( C) Binding of His6-tagged ribosomal protein S1 to 100 pM 32P-labeled PK1L and PK3L SsrA variants.	bind
48328	3	914	7	NULL	NULL	0	NULL	S1	GP		is a type of					ribosomal protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_6_3040_s_132	11248028	( B) Binding curve generated from data in  A. ( C) Binding of His6-tagged ribosomal protein S1 to 100 pM 32P-labeled PK1L and PK3L SsrA variants.	bind
218	1	915	6	10	NULL	0	NULL	SPP	NULL		bind	NULL				HEK293 EDG-1 cells	NULL				NULL		NULL	NULL	NULL	NULL	gw60_science_279_5356_1552_s_93	9488656	( B) Binding isotherm of [32]SPP to HEK293 EDG-1 cells.	bind
48329	1	915	7	NULL	NULL	0	NULL	SPP	GP		bind					HEK293 EDG-1 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_science_279_5356_1552_s_93	9488656	( B) Binding isotherm of [32]SPP to HEK293 EDG-1 cells.	bind
219	1	916	6	10	NULL	0	NULL	Ets proteins	NULL	C.elegans	bind	NULL				EBS probe	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_20_4154_s_263	11600704	( B) Binding of  C.elegans Ets proteins to the EBS probe.	bind
48330	1	916	7	NULL	NULL	0	NULL	Ets protein	GP	C.elegans	bind					EBS probe	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_20_4154_s_263	11600704	( B) Binding of  C.elegans Ets proteins to the EBS probe.	bind
220	1	917	6	NULL	NULL	0	NULL	A1	NULL		bind	NULL				CE4	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_18_7_1939_s_184	10202157	( B) Binding of A1 to CE4 or CE4m.	bind
221	2	917	6	NULL	NULL	0	NULL	A1	NULL		bind	NULL				CE4m	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_18_7_1939_s_184	10202157	( B) Binding of A1 to CE4 or CE4m.	bind
48331	1	917	7	NULL	NULL	0	NULL	 A1	GP		bind					CE4	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_7_1939_s_184	10202157	( B) Binding of A1 to CE4 or CE4m.	bind
48332	2	917	7	NULL	NULL	0	NULL	A1	GP		bind					CE4m	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_7_1939_s_184	10202157	( B) Binding of A1 to CE4 or CE4m.	bind
223	1	918	6	10	NULL	0	NULL	APE1	NULL		bind	NULL				AP-dsDNA	NULL				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_5_1552_s_208	16540594	( B) Binding of APE1 and its mutant proteins to the dsDNA containing an AP site (AP-dsDNA).	bind
225	2	918	6	10	NULL	0	NULL	APE1	NULL	mutant	bind	NULL				AP-dsDNA	NULL				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_5_1552_s_208	16540594	( B) Binding of APE1 and its mutant proteins to the dsDNA containing an AP site (AP-dsDNA).	bind
51439	3	918	6	10	NULL	0	NULL	AP-dsDNA	NULL		is	NULL				dsDNA containing an AP site	NULL				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_34_5_1552_s_208	16540594	( B) Binding of APE1 and its mutant proteins to the dsDNA containing an AP site (AP-dsDNA).	bind
48333	1	918	7	NULL	NULL	0	NULL	APE1 	GP		bind					AP-dsDNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_5_1552_s_208	16540594	( B) Binding of APE1 and its mutant proteins to the dsDNA containing an AP site (AP-dsDNA).	bind
48334	2	918	7	NULL	NULL	0	NULL	APE1 	GP	mutant	bind					AP-dsDNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_5_1552_s_208	16540594	( B) Binding of APE1 and its mutant proteins to the dsDNA containing an AP site (AP-dsDNA).	bind
48335	3	918	7	NULL	NULL	0	NULL	AP-dsDNA	NucleicAcid		is					dsDNA	NucleicAcid			AP site containing	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_5_1552_s_208	16540594	( B) Binding of APE1 and its mutant proteins to the dsDNA containing an AP site (AP-dsDNA).	bind
228	1	919	6	NULL	NULL	0	NULL	Bcl-w	NULL		bind	NULL				BimLdeltaC27	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_22_7_1497_s_135	12660157	( B) Binding of Bcl-w to BimLdeltaC27 fits a 1:1 model.	bind
48336	1	919	7	NULL	NULL	0	NULL	Bcl-w	GP		bind					BimLdeltaC27	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_22_7_1497_s_135	12660157	( B) Binding of Bcl-w to BimLdeltaC27 fits a 1:1 model.	bind
229	1	920	6	10	NULL	0	NULL	c-Rel	NULL		bind	NULL				Il12b	NULL	endogenous		Promoter	NULL	bone marrow-derived macrophages stimulated with LPS + IFN-gamma	NULL	NULL	NULL	NULL	gw70_genesdev_19_18_2138_s_223	16166378	( B) Binding of c-Rel and p65 to the endogenous  Il12b promoter in bone marrow-derived macrophages stimulated with LPS + IFN-gamma was monitored by ChIP.	bind
233	2	920	6	10	NULL	0	NULL	p65	NULL		bind	NULL				Il12b	NULL	endogenous		Promoter	NULL	bone marrow-derived macrophages stimulated with LPS + IFN-gamma	NULL	NULL	NULL	NULL	gw70_genesdev_19_18_2138_s_223	16166378	( B) Binding of c-Rel and p65 to the endogenous  Il12b promoter in bone marrow-derived macrophages stimulated with LPS + IFN-gamma was monitored by ChIP.	bind
48340	1	920	7	NULL	NULL	0	NULL	 c-Rel	GP		bind					Il12b	GP	endogenous		promoter	NULL	bone marrow-derived macrophages stimulated with LPS + IFN-gamma	NULL	NULL	NULL	NULL	gw70_genesdev_19_18_2138_s_223	16166378	( B) Binding of c-Rel and p65 to the endogenous  Il12b promoter in bone marrow-derived macrophages stimulated with LPS + IFN-gamma was monitored by ChIP.	bind
48341	2	920	7	NULL	NULL	0	NULL	p65	GP		bind					Il12b	GP	endogenous		promoter	NULL	bone marrow-derived macrophages stimulated with LPS + IFN-gamma	NULL	NULL	NULL	NULL	gw70_genesdev_19_18_2138_s_223	16166378	( B) Binding of c-Rel and p65 to the endogenous  Il12b promoter in bone marrow-derived macrophages stimulated with LPS + IFN-gamma was monitored by ChIP.	bind
234	1	921	6	10	NULL	0	NULL	CBP	NULL		bind	NULL				SRC1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_1_232_s_180	9427757	( B) Binding of CBP to GST fusions of SRC1.	bind
51440	2	921	6	10	NULL	0	NULL	SRC1	NULL		is a type of	NULL				GST fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_17_1_232_s_180	9427757	( B) Binding of CBP to GST fusions of SRC1.	bind
48342	1	921	7	NULL	NULL	0	NULL	CBP	GP		bind					SRC1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_1_232_s_180	9427757	( B) Binding of CBP to GST fusions of SRC1.	bind
48343	2	921	7	NULL	NULL	0	NULL	SRC1	GP		is a type of					GST fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_1_232_s_180	9427757	( B) Binding of CBP to GST fusions of SRC1.	bind
235	1	922	6	NULL	NULL	0	NULL	cdc45p	NULL		bind	NULL				Mcm2p	NULL				NULL	chromatin	0	NULL	NULL	NULL	gw60_science_280_5363_593_s_99	9554851	( B) Binding of Cdc45p to Mcm2p on chromatin.	bind
48344	1	922	7	NULL	NULL	0	NULL	Cdc45p	GP		bind					Mcm2p	GP				NULL	chromatin	NULL	NULL	NULL	NULL	gw60_science_280_5363_593_s_99	9554851	( B) Binding of Cdc45p to Mcm2p on chromatin.	bind
236	1	923	6	10	NULL	0	NULL	Cdc6	NULL		bind	NULL				ORC	NULL				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_13_3293_s_78	11432816	( B) Binding of Cdc6 and RLF-B/Cdt1 onto ORC.	bind
51441	2	923	6	10	NULL	0	NULL	RLF-B/Cdt1	NULL		bind	NULL				ORC	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_20_13_3293_s_78	11432816	( B) Binding of Cdc6 and RLF-B/Cdt1 onto ORC.	bind
48345	1	923	7	NULL	NULL	0	NULL	Cdc6 	GP		bind					ORC	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_13_3293_s_78	11432816	( B) Binding of Cdc6 and RLF-B/Cdt1 onto ORC.	bind
48346	2	923	7	NULL	NULL	0	NULL	RLF-B/Cdt1 	GP		bind					ORC	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_13_3293_s_78	11432816	( B) Binding of Cdc6 and RLF-B/Cdt1 onto ORC.	bind
237	1	924	6	NULL	NULL	0	NULL	cFos	NULL		bind	NULL				collagenase-1 gene	NULL			colA element	NULL		0	NULL	NULL	NULL	gw60_embo_20_21_6071_s_82	11689447	( B) Binding of cFos to the colA element of the collagenase-1 gene.	bind
48347	1	924	7	NULL	NULL	0	NULL	cFos	GP		bind					collagenase-1 gene	GP			colA element	NULL		NULL	NULL	NULL	NULL	gw60_embo_20_21_6071_s_82	11689447	( B) Binding of cFos to the colA element of the collagenase-1 gene.	bind
238	1	925	6	10	NULL	0	NULL	IgA	NULL	control	bind	NULL				R2 cells	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_105_12_1731_s_172	10862788	( b) Binding of control IgA and T15 to R2 cells.	bind
239	2	925	6	NULL	NULL	0	NULL	T15	NULL		bind	NULL				R2 cells	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_105_12_1731_s_172	10862788	( b) Binding of control IgA and T15 to R2 cells.	bind
48348	1	925	7	NULL	NULL	0	NULL	IgA 	GP	control	bind					R2 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_105_12_1731_s_172	10862788	( b) Binding of control IgA and T15 to R2 cells.	bind
48349	2	925	7	NULL	NULL	0	NULL	T15	GP		bind					R2 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_105_12_1731_s_172	10862788	( b) Binding of control IgA and T15 to R2 cells.	bind
240	1	927	6	NULL	NULL	0	NULL	CYP2E1 	NULL		bind	NULL				FANCG	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_23_1_67_s_110	11756225	( B) Binding of CYP2E1 to FANCG.	bind
48350	1	927	7	NULL	NULL	0	NULL	CYP2E1	GP		bind					FANCG	GP				NULL		NULL	NULL	NULL	NULL	gw60_carcinogenesis_23_1_67_s_110	11756225	( B) Binding of CYP2E1 to FANCG.	bind
241	1	928	6	NULL	NULL	0	NULL	Dsg1	NULL		bind	NULL				ETA Cmu	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_110_1_53_s_177	12093888	( b) Binding of Dsg1 with ETA Cmu and ETA Amu.	bind
242	2	928	6	NULL	NULL	0	NULL	Dsg1	NULL		bind	NULL				ETA Amu	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_110_1_53_s_177	12093888	( b) Binding of Dsg1 with ETA Cmu and ETA Amu.	bind
48351	1	928	7	NULL	NULL	0	NULL	Dsg1	GP		bind					ETA Cmu 	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_110_1_53_s_177	12093888	( b) Binding of Dsg1 with ETA Cmu and ETA Amu.	bind
48352	2	928	7	NULL	NULL	0	NULL	Dsg1	GP		bind					ETA Amu	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_110_1_53_s_177	12093888	( b) Binding of Dsg1 with ETA Cmu and ETA Amu.	bind
243	1	929	6	NULL	NULL	0	NULL	E12	NULL		bind	NULL				p300	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_6_820_s_82	9512516	( B) Binding of E12 to p300.	bind
48353	1	929	7	NULL	NULL	0	NULL	E12 	GP		bind					p300	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_6_820_s_82	9512516	( B) Binding of E12 to p300.	bind
244	1	930	6	10	NULL	0	NULL	PKCI-r RNA fragment	NULL		bind	NULL				ASF/SF2	NULL	purified;;baculovirus-expressed			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_5_594_s_225	11877379	( B) Binding of each of the five  PKCI-r RNA fragments to ASF/SF2 was then assessed using increasing amounts (0, 17, 50, and 150 ng) of purified baculovirus-expressed ASF/SF2 in gel shift assays.	bind
48354	1	930	7	NULL	NULL	0	NULL	PKCI-r RNA fragments	NucleicAcid		bind					ASF/SF2	GP	purified;;baculovirus-expressed			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_5_594_s_225	11877379	( B) Binding of each of the five  PKCI-r RNA fragments to ASF/SF2 was then assessed using increasing amounts (0, 17, 50, and 150 ng) of purified baculovirus-expressed ASF/SF2 in gel shift assays.	bind
245	1	931	6	10	NULL	0	NULL	Eps15	NULL		bind	NULL				NPF-containing peptides	NULL				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_17_2239_s_104	9303539	( B) Binding of Eps15 to GST fusions encompassing NPF-containing peptides.	bind
51442	2	931	6	10	NULL	0	NULL	NPF-containing peptides	NULL		is a type of	NULL				GST fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_11_17_2239_s_104	9303539	( B) Binding of Eps15 to GST fusions encompassing NPF-containing peptides.	bind
48355	1	931	7	NULL	NULL	0	NULL	 Eps15 	GP		bind					NPF-containing peptides	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_17_2239_s_104	9303539	( B) Binding of Eps15 to GST fusions encompassing NPF-containing peptides.	bind
48356	2	931	7	NULL	NULL	0	NULL	NPF-containing peptides	GP		is a type of					GST fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_17_2239_s_104	9303539	( B) Binding of Eps15 to GST fusions encompassing NPF-containing peptides.	bind
246	1	933	6	NULL	NULL	0	NULL	bacteria	NULL	FimH-expressing	bind	NULL				CHO cells	NULL	CD48-expressing			NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_14_8110_s_140	10393956	( B) Binding of FimH-expressing bacteria to CD48-expressing CHO cells and control CHO cells.	bind
51444	2	933	6	10	NULL	0	NULL	bacteria	NULL	FimH-expressing	bind	NULL				CHO cells	NULL	control			NULL		0	NULL	NULL	NULL	gw60_pnas_96_14_8110_s_140	10393956	( B) Binding of FimH-expressing bacteria to CD48-expressing CHO cells and control CHO cells.	bind
48357	1	933	7	NULL	NULL	0	NULL	bacteria	Organism		express					FimH	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_14_8110_s_140	10393956	( B) Binding of FimH-expressing bacteria to CD48-expressing CHO cells and control CHO cells.	bind
48358	2	933	7	NULL	NULL	0	NULL	CHO cells	Cell		express					CD48	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_14_8110_s_140	10393956	( B) Binding of FimH-expressing bacteria to CD48-expressing CHO cells and control CHO cells.	bind
48359	3	933	7	NULL	NULL	0	NULL	statement 1	Process		bind					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_14_8110_s_140	10393956	( B) Binding of FimH-expressing bacteria to CD48-expressing CHO cells and control CHO cells.	bind
51443	4	933	7	NULL	NULL	0	NULL	statement 1	Process		bind					CHO cells	Cell	control			NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_14_8110_s_140	10393956	( B) Binding of FimH-expressing bacteria to CD48-expressing CHO cells and control CHO cells.	bind
247	1	934	6	NULL	NULL	0	NULL	gp5/trx	NULL		bind	NULL				gp4	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_14_5096_s_100	15795374	( B) Binding of gp5/trx to gp4 or gp4-Cdelta17.	bind
248	2	934	6	NULL	NULL	0	NULL	gp5/trx	NULL		bind	NULL				gp4-Cdelta17	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_14_5096_s_100	15795374	( B) Binding of gp5/trx to gp4 or gp4-Cdelta17.	bind
51445	3	934	6	10	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_14_5096_s_100	15795374	( B) Binding of gp5/trx to gp4 or gp4-Cdelta17.	bind
48361	1	934	7	NULL	NULL	0	NULL	gp5/trx	GP		bind					gp4	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_14_5096_s_100	15795374	( B) Binding of gp5/trx to gp4 or gp4-Cdelta17.	bind
48362	2	934	7	NULL	NULL	0	NULL	gp5/trx	GP		bind					gp4-Cdelta17	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_14_5096_s_100	15795374	( B) Binding of gp5/trx to gp4 or gp4-Cdelta17.	bind
48363	3	934	7	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_14_5096_s_100	15795374	( B) Binding of gp5/trx to gp4 or gp4-Cdelta17.	bind
249	1	935	6	NULL	NULL	0	NULL	Griseofulvin	NULL		bind	NULL				Tubulin	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_28_9878_s_150	15985553	( B) Binding of griseofulvin to tubulin.	bind
48364	1	935	7	NULL	NULL	0	NULL	 griseofulvin	GP		bind					tubulin	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_28_9878_s_150	15985553	( B) Binding of griseofulvin to tubulin.	bind
250	1	936	6	10	NULL	0	NULL	GST	NULL		bind	NULL				homopolynucleotides	NULL	radiolabeled			NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_21_6795_s_201	16396833	( B) Binding of GST and GST - MPP6 fusion proteins to radiolabelled homopolynucleotides  was analysed as described above and the bound RNAs were quantified in a scintillation  counter.	bind
251	2	936	6	10	NULL	0	NULL	GST - MPP6	NULL		bind	NULL				homopolynucleotides	NULL	radiolabeled			NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_21_6795_s_201	16396833	( B) Binding of GST and GST - MPP6 fusion proteins to radiolabelled homopolynucleotides  was analysed as described above and the bound RNAs were quantified in a scintillation  counter.	bind
51446	3	936	6	10	NULL	0	NULL	GST - MPP6	NULL		is a type of	NULL				fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_21_6795_s_201	16396833	( B) Binding of GST and GST - MPP6 fusion proteins to radiolabelled homopolynucleotides  was analysed as described above and the bound RNAs were quantified in a scintillation  counter.	bind
48365	1	936	7	NULL	NULL	0	NULL	GST	Chemical		bind					 homopolynucleotides	NucleicAcid	 radiolabelled 			NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_21_6795_s_201	16396833	( B) Binding of GST and GST - MPP6 fusion proteins to radiolabelled homopolynucleotides  was analysed as described above and the bound RNAs were quantified in a scintillation  counter.	bind
48366	2	936	7	NULL	NULL	0	NULL	GST - MPP6	GP		bind					homopolynucleotides	NucleicAcid	radiolabelled			NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_21_6795_s_201	16396833	( B) Binding of GST and GST - MPP6 fusion proteins to radiolabelled homopolynucleotides  was analysed as described above and the bound RNAs were quantified in a scintillation  counter.	bind
48367	3	936	7	NULL	NULL	0	NULL	GST - MPP6	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_21_6795_s_201	16396833	( B) Binding of GST and GST - MPP6 fusion proteins to radiolabelled homopolynucleotides  was analysed as described above and the bound RNAs were quantified in a scintillation  counter.	bind
252	1	937	6	NULL	NULL	0	NULL	GST-Dsk2p	NULL		bind	NULL				Ub	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_2_745_s_102	11805328	( B) Binding of GST-Dsk2p to Ub.	bind
48368	1	937	7	NULL	NULL	0	NULL	GST-Dsk2p 	GP		bind					Ub	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_2_745_s_102	11805328	( B) Binding of GST-Dsk2p to Ub.	bind
253	1	938	6	NULL	NULL	0	NULL	GST-Rup1	NULL		 bind	NULL				Rsp5 proteins	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_24_13_2414_s_122	15933713	( B) Binding of GST-Rup1 to Rsp5 proteins.	bind
48369	1	938	7	NULL	NULL	0	NULL	GST-Rup1	GP		bind					Rsp5 protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_13_2414_s_122	15933713	( B) Binding of GST-Rup1 to Rsp5 proteins.	bind
254	1	939	6	NULL	NULL	0	NULL	GST-Rup1	NULL		bind	NULL				Ubp2 proteins	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_24_13_2414_s_133	15933713	( B) Binding of GST-Rup1 to Ubp2 proteins.	bind
48370	1	939	7	NULL	NULL	0	NULL	GST-Rup1	GP		bind					Ubp2 protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_13_2414_s_133	15933713	( B) Binding of GST-Rup1 to Ubp2 proteins.	bind
255	1	940	6	10	NULL	0	NULL	Hop1	NULL		bind	NULL				48 bp duplex DNA	NULL				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_32_8_2378_s_77	15115800	( B) Binding of Hop1 to 48 bp duplex DNA containing a mismatched G/G region.	bind
51447	2	940	6	10	NULL	0	NULL	48 bp duplex DNA	NULL		contains	NULL					NULL			mismatched G/G region	NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_32_8_2378_s_77	15115800	( B) Binding of Hop1 to 48 bp duplex DNA containing a mismatched G/G region.	bind
48371	1	940	7	NULL	NULL	0	NULL	Hop1	GP		bind					duplex DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_32_8_2378_s_77	15115800	( B) Binding of Hop1 to 48 bp duplex DNA containing a mismatched G/G region.	bind
51448	2	940	7	NULL	NULL	0	NULL	48 bp duplex DNA	NucleicAcid		contains									mismatched G/G region	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_32_8_2378_s_77	15115800	( B) Binding of Hop1 to 48 bp duplex DNA containing a mismatched G/G region.	bind
256	1	941	6	NULL	NULL	0	NULL	IAPP	NULL		bind	NULL				IAPP-GI	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_103_7_2046_s_128	16467158	( B) Binding of IAPP to IAPP-GI as assessed by fluorescence spectroscopy:	bind
48372	1	941	7	NULL	NULL	0	NULL	IAPP	GP		bind					IAPP-GI	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_7_2046_s_128	16467158	( B) Binding of IAPP to IAPP-GI as assessed by fluorescence spectroscopy:	bind
257	1	942	6	NULL	NULL	0	NULL	IMP1	NULL		bind	NULL				ARS RNA	NULL				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_226	16356927	( B) Binding of IMP1 to the ARS RNA. [35]methionine labeled 6x His-tagged IMP1, PABP, UNR and beta-galactosidase were expressed in  E. coliand purified by Ni-NTA agarose as described in Materials and Methods.	bind
48373	1	942	7	NULL	NULL	0	NULL	IMP1	GP		bind					ARS RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_226	16356927	( B) Binding of IMP1 to the ARS RNA. [35]methionine labeled 6x His-tagged IMP1, PABP, UNR and beta-galactosidase were expressed in  E. coliand purified by Ni-NTA agarose as described in Materials and Methods.	bind
258	1	943	6	NULL	NULL	0	NULL	JNK	NULL		bind	NULL				NFAT4	NULL		NH2-terminal region		NULL		0	NULL	NULL	NULL	gw60_science_278_5343_1638_s_42	9374467	( B) Binding of JNK to the NH2-terminal region of NFAT4.	bind
48374	1	943	7	NULL	NULL	0	NULL	JNK	GP		bind					NFAT4	GP		NH2-terminal region		NULL		NULL	NULL	NULL	NULL	gw60_science_278_5343_1638_s_42	9374467	( B) Binding of JNK to the NH2-terminal region of NFAT4.	bind
259	1	944	6	NULL	NULL	0	NULL	JNK1	NULL		bind	NULL				GST	NULL				NULL		0	NULL	NULL	NULL	gw60_science_277_5326_693_s_77	9235893	( B) Binding of JNK1 to GST and GST-JIP-1 (residues 127 to 281) was examined in the absence and presence of synthetic peptides (64 mug/ml).	bind
260	2	944	6	10	NULL	0	NULL	JNK1	NULL		bind	NULL				GST-JIP-1	NULL		residues 127 to 281		NULL		NULL	NULL	NULL	NULL	gw60_science_277_5326_693_s_77	9235893	( B) Binding of JNK1 to GST and GST-JIP-1 (residues 127 to 281) was examined in the absence and presence of synthetic peptides (64 mug/ml).	bind
48375	1	944	7	NULL	NULL	0	NULL	 JNK1	GP		bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_277_5326_693_s_77	9235893	( B) Binding of JNK1 to GST and GST-JIP-1 (residues 127 to 281) was examined in the absence and presence of synthetic peptides (64 mug/ml).	bind
48376	2	944	7	NULL	NULL	0	NULL	 JNK1	GP		bind					GST-JIP-1	GP		residues 127 to 281		NULL		NULL	NULL	NULL	NULL	gw60_science_277_5326_693_s_77	9235893	( B) Binding of JNK1 to GST and GST-JIP-1 (residues 127 to 281) was examined in the absence and presence of synthetic peptides (64 mug/ml).	bind
262	1	946	6	NULL	NULL	0	NULL	MafK	NULL		bind	NULL				ho-1 E2	NULL			enhancer	NULL		0	NULL	NULL	NULL	gw70_embo_23_13_2544_s_231	15175654	( B) Binding of MafK or Nrf2 to the  ho-1 E2 enhancer was examined as in	bind
263	2	946	6	NULL	NULL	0	NULL	Nrf2	NULL		bind	NULL				ho-1 E2	NULL			enhancer	NULL		0	NULL	NULL	NULL	gw70_embo_23_13_2544_s_231	15175654	( B) Binding of MafK or Nrf2 to the  ho-1 E2 enhancer was examined as in	bind
48378	1	946	7	NULL	NULL	0	NULL	MafK	GP		bind					ho-1 E2	GP			enhancer	NULL		NULL	NULL	NULL	NULL	gw70_embo_23_13_2544_s_231	15175654	( B) Binding of MafK or Nrf2 to the  ho-1 E2 enhancer was examined as in	bind
48379	2	946	7	NULL	NULL	0	NULL	Nrf2	GP		bind					ho-1 E2 	GP			enhancer	NULL		NULL	NULL	NULL	NULL	gw70_embo_23_13_2544_s_231	15175654	( B) Binding of MafK or Nrf2 to the  ho-1 E2 enhancer was examined as in	bind
264	1	947	6	NULL	NULL	0	NULL	MAp18	NULL		bind	NULL				TIP47	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_103_40_14947_s_79	17003132	( B) Binding of MAp18 to TIP47 in a cell lysate-binding assay.	bind
48380	1	947	7	NULL	NULL	0	NULL	MAp18	GP		bind					TIP47	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_40_14947_s_79	17003132	( B) Binding of MAp18 to TIP47 in a cell lysate-binding assay.	bind
265	1	948	6	NULL	NULL	0	NULL	mSIN3A	NULL		bind	NULL				CTCF	NULL				NULL	In vitro	0	NULL	NULL	NULL	gw60_nucleicacidsres_28_8_1707_s_133	10734189	( B) Binding of mSIN3A deletions to CTCF  in vitro.	bind
48381	1	948	7	NULL	NULL	0	NULL	mSIN3A	GP	deletion	bind					CTCF	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_8_1707_s_133	10734189	( B) Binding of mSIN3A deletions to CTCF  in vitro.	bind
266	1	949	6	NULL	NULL	0	NULL	mtHsp70	NULL		bind	NULL				peptide substrate	NULL				NULL		0	NULL	NULL	NULL	gw60_science_300_5616_139_s_39	12677068	( B) Binding of mtHsp70 to peptide substrate.	bind
48382	1	949	7	NULL	NULL	0	NULL	mtHsp70	GP		bind					peptide substrate	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5616_139_s_39	12677068	( B) Binding of mtHsp70 to peptide substrate.	bind
267	1	950	6	NULL	NULL	0	NULL	MyoD	NULL		bind	NULL				DNA	NULL			E-box	NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_9_2887_s_247	15908587	( B) Binding of MyoD to E-box DNA.	bind
48383	1	950	7	NULL	NULL	0	NULL	MyoD	GP		bind					DNA	NucleicAcid			E-box	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_9_2887_s_247	15908587	( B) Binding of MyoD to E-box DNA.	bind
268	1	951	6	NULL	NULL	0	NULL	myostatin	NULL		bind	NULL				lectin	NULL	lentil			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_16_9306_s_54	11459935	( b) Binding of myostatin to lentil lectin.	bind
48384	1	951	7	NULL	NULL	0	NULL	myostatin	GP		bind					 lectin	GP	lentil			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_16_9306_s_54	11459935	( b) Binding of myostatin to lentil lectin.	bind
269	1	952	6	NULL	NULL	0	NULL	NS1	NULL		bind	NULL				p85beta	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_103_38_14194_s_129	16963558	( b) Binding of NS1 to p85beta requires Y89 and M93.	bind
270	2	952	6	NULL	NULL	0	NULL	Statement 1	NULL		requires	NULL				Y89	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_103_38_14194_s_129	16963558	( b) Binding of NS1 to p85beta requires Y89 and M93.	bind
271	3	952	6	NULL	NULL	0	NULL	Statement 1	NULL		requires	NULL				M93	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_103_38_14194_s_129	16963558	( b) Binding of NS1 to p85beta requires Y89 and M93.	bind
48385	1	952	7	NULL	NULL	0	NULL	NS1	GP		bind					p85beta	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_38_14194_s_129	16963558	( b) Binding of NS1 to p85beta requires Y89 and M93.	bind
48386	2	952	7	NULL	NULL	0	NULL	statement 1	Process		requires					Y89	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_38_14194_s_129	16963558	( b) Binding of NS1 to p85beta requires Y89 and M93.	bind
48387	3	952	7	NULL	NULL	0	NULL	statement 1	Process		requires					M93	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_38_14194_s_129	16963558	( b) Binding of NS1 to p85beta requires Y89 and M93.	bind
331	1	953	6	10	NULL	0	NULL	OGG1 enzymes	NULL		bind	NULL				substrate	NULL		abasic site		NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_5_1620_s_169	16549874	( B) Binding of OGG1 enzymes to an abasic site substrate after adding APE1 was measured  by EMSA.	bind
48388	1	953	7	NULL	NULL	0	NULL	OGG1 enzyme	GP		bind					substrate	GP		abasic site 		NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_5_1620_s_169	16549874	( B) Binding of OGG1 enzymes to an abasic site substrate after adding APE1 was measured  by EMSA.	bind
332	1	954	6	NULL	NULL	0	NULL	PCNA	NULL	binding of 	require	NULL				ATP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_14_3811_s_166	10899134	( B) Binding of PCNA requires ATP (lanes 2 and 3) and binding of FEN1 requires PCNA (lanes 1 and 4).	bind
333	2	954	6	NULL	NULL	0	NULL	FEN1	NULL	binding of 	require	NULL				PCNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_14_3811_s_166	10899134	( B) Binding of PCNA requires ATP (lanes 2 and 3) and binding of FEN1 requires PCNA (lanes 1 and 4).	bind
48389	1	954	7	NULL	NULL	0	NULL	PCNA	GP	binding of	requires					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_14_3811_s_166	10899134	( B) Binding of PCNA requires ATP (lanes 2 and 3) and binding of FEN1 requires PCNA (lanes 1 and 4).	bind
48390	2	954	7	NULL	NULL	0	NULL	FEN1	GP	binding of	requires					PCNA	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_14_3811_s_166	10899134	( B) Binding of PCNA requires ATP (lanes 2 and 3) and binding of FEN1 requires PCNA (lanes 1 and 4).	bind
334	1	955	6	10	NULL	0	NULL	PI4,5P2	NULL		bind	NULL					NULL		ABD		NULL		NULL	NULL	NULL	NULL	gw60_embo_19_23_6331_s_223	11101506	( B) Binding of PI4,5P2 to the ABD induces a conformational change that switches on titin binding by making the EF3/4 region available for binding to Z-repeats (ZR7).	bind
336	2	955	6	10	NULL	0	NULL	Statement 1	NULL		induce	NULL					NULL	conformation change of 	ABD		NULL		NULL	NULL	NULL	NULL	gw60_embo_19_23_6331_s_223	11101506	( B) Binding of PI4,5P2 to the ABD induces a conformational change that switches on titin binding by making the EF3/4 region available for binding to Z-repeats (ZR7).	bind
340	3	955	6	NULL	NULL	0	NULL	Statement 2	NULL		makes available	NULL				EF3/4 region	NULL				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_23_6331_s_223	11101506	( B) Binding of PI4,5P2 to the ABD induces a conformational change that switches on titin binding by making the EF3/4 region available for binding to Z-repeats (ZR7).	bind
609	4	955	6	NULL	NULL	0	NULL		NULL		bind	NULL		EF3/4 region		titin	NULL	Z-repeats			NULL		0	NULL	NULL	NULL	gw60_embo_19_23_6331_s_223	11101506	( B) Binding of PI4,5P2 to the ABD induces a conformational change that switches on titin binding by making the EF3/4 region available for binding to Z-repeats (ZR7).	bind
610	5	955	6	NULL	NULL	0	NULL	Statement 3	NULL		allows	NULL				Statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_19_23_6331_s_223	11101506	( B) Binding of PI4,5P2 to the ABD induces a conformational change that switches on titin binding by making the EF3/4 region available for binding to Z-repeats (ZR7).	bind
611	6	955	6	NULL	NULL	0	NULL	statement 5 	NULL		turns on	NULL				titin	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_embo_19_23_6331_s_223	11101506	( B) Binding of PI4,5P2 to the ABD induces a conformational change that switches on titin binding by making the EF3/4 region available for binding to Z-repeats (ZR7).	bind
612	7	955	6	NULL	NULL	0	NULL	ZR7	NULL		is	NULL				Z repeats	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_19_23_6331_s_223	11101506	( B) Binding of PI4,5P2 to the ABD induces a conformational change that switches on titin binding by making the EF3/4 region available for binding to Z-repeats (ZR7).	bind
48391	1	955	7	NULL	NULL	0	NULL	PI4,5P2	Chemical		bind								ABD		NULL		NULL	NULL	NULL	NULL	gw60_embo_19_23_6331_s_223	11101506	( B) Binding of PI4,5P2 to the ABD induces a conformational change that switches on titin binding by making the EF3/4 region available for binding to Z-repeats (ZR7).	bind
48392	2	955	7	NULL	NULL	0	NULL	titin	GP		bind			EF3/4 region		ZR7	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_23_6331_s_223	11101506	( B) Binding of PI4,5P2 to the ABD induces a conformational change that switches on titin binding by making the EF3/4 region available for binding to Z-repeats (ZR7).	bind
48393	3	955	7	NULL	NULL	0	NULL	statement 1	Process		induce					conformational change	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_23_6331_s_223	11101506	( B) Binding of PI4,5P2 to the ABD induces a conformational change that switches on titin binding by making the EF3/4 region available for binding to Z-repeats (ZR7).	bind
48394	4	955	7	NULL	NULL	0	NULL	statement 3	Process		switches on					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_23_6331_s_223	11101506	( B) Binding of PI4,5P2 to the ABD induces a conformational change that switches on titin binding by making the EF3/4 region available for binding to Z-repeats (ZR7).	bind
48395	5	955	7	NULL	NULL	0	NULL	ZR7	GP		is a type of					Z-repeat	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_23_6331_s_223	11101506	( B) Binding of PI4,5P2 to the ABD induces a conformational change that switches on titin binding by making the EF3/4 region available for binding to Z-repeats (ZR7).	bind
341	1	956	6	10	NULL	0	NULL	EGSs	NULL		bind	NULL				PR mRNA substrate	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_26_14831_s_111	11742095	( B) Binding of PR mRNA substrate by EGSs.	bind
48396	1	956	7	NULL	NULL	0	NULL	EGSs	GP		bind					PR mRNA substrate	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_26_14831_s_111	11742095	( B) Binding of PR mRNA substrate by EGSs.	bind
342	1	957	6	10	NULL	0	NULL	Ras	NULL		bind	NULL		A59G		Raf kinase	NULL		RBD		NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_19_12138_s_133	12213964	( B) Binding of RasA59G to the Ras-binding domain (RBD) of the Raf kinase.	bind
51449	2	957	6	10	NULL	0	NULL	RBD	NULL		is	NULL				Ras-binding domain	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_19_12138_s_133	12213964	( B) Binding of RasA59G to the Ras-binding domain (RBD) of the Raf kinase.	bind
48397	1	957	7	NULL	NULL	0	NULL	Ras	GP		bind			A59G		Raf kinase	GP		RBD		NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_19_12138_s_133	12213964	( B) Binding of RasA59G to the Ras-binding domain (RBD) of the Raf kinase.	bind
48398	2	957	7	NULL	NULL	0	NULL	RBD	GP		is					Ras-binding domain	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_19_12138_s_133	12213964	( B) Binding of RasA59G to the Ras-binding domain (RBD) of the Raf kinase.	bind
344	1	958	6	NULL	NULL	0	NULL	RPA-A	NULL		bind	NULL				CPD/AA-10 duplex	NULL				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_31_16_4747_s_128	12907715	( B) Binding of RPA-A to the CPD/AA-10 duplex as a function of DNA concentration in the  absence (upper) and presence (lower) of equimolar XPA-MBD.	bind
48399	1	958	7	NULL	NULL	0	NULL	RPA-A	GP		bind					CPD/AA-10 duplex	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_16_4747_s_128	12907715	( B) Binding of RPA-A to the CPD/AA-10 duplex as a function of DNA concentration in the  absence (upper) and presence (lower) of equimolar XPA-MBD.	bind
346	1	959	6	NULL	NULL	0	NULL	RPA-A 	NULL		bind	NULL				CPD/AA-10 duplex	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_16_4747_s_128	12907715	( B) Binding of RPA-A to the CPD/AA-10 duplex as a function of DNA concentration in the absence (upper) and presence (lower) of equimolar XPA-MBD.	bind
348	1	960	6	NULL	NULL	0	NULL	Salp	NULL		bind	NULL				p85	NULL		SH3 domain		NULL		0	NULL	NULL	NULL	gw60_gene_240_1_133_s_253	10564820	( B) Binding of Salp  to the p85 SH3 domain.	bind
48400	1	960	7	NULL	NULL	0	NULL	 Salp	GP		bind					p85	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_gene_240_1_133_s_253	10564820	( B) Binding of Salp  to the p85 SH3 domain.	bind
349	1	961	6	NULL	NULL	0	NULL	Sec17p	NULL		bind	NULL				vacuole	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_140_1_61_s_216	9425154	( B) Binding of Sec17p and Sec18p to the vacuole is independent of the Nyv1p and Vam3p.	bind
351	2	961	6	NULL	NULL	0	NULL	Sec18p	NULL		bind	NULL				vacuole	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_140_1_61_s_216	9425154	( B) Binding of Sec17p and Sec18p to the vacuole is independent of the Nyv1p and Vam3p.	bind
352	3	961	6	NULL	NULL	0	NULL	Statement 1	NULL		is independent of	NULL				Nyv1p	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_140_1_61_s_216	9425154	( B) Binding of Sec17p and Sec18p to the vacuole is independent of the Nyv1p and Vam3p.	bind
353	4	961	6	NULL	NULL	0	NULL	statement 2	NULL		is independent of	NULL				Nyv1p	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_140_1_61_s_216	9425154	( B) Binding of Sec17p and Sec18p to the vacuole is independent of the Nyv1p and Vam3p.	bind
354	5	961	6	NULL	NULL	0	NULL	Statement 1	NULL		is independent of	NULL				Vam3p	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_140_1_61_s_216	9425154	( B) Binding of Sec17p and Sec18p to the vacuole is independent of the Nyv1p and Vam3p.	bind
355	6	961	6	NULL	NULL	0	NULL	statement 2	NULL		is independent of	NULL				Vam3p	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_140_1_61_s_216	9425154	( B) Binding of Sec17p and Sec18p to the vacuole is independent of the Nyv1p and Vam3p.	bind
48401	1	961	7	NULL	NULL	0	NULL	Sec17p	GP		bind 					vacuole	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_140_1_61_s_216	9425154	( B) Binding of Sec17p and Sec18p to the vacuole is independent of the Nyv1p and Vam3p.	bind
48402	2	961	7	NULL	NULL	0	NULL	Sec18p	GP		bind					vacuole	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_140_1_61_s_216	9425154	( B) Binding of Sec17p and Sec18p to the vacuole is independent of the Nyv1p and Vam3p.	bind
48403	3	961	7	NULL	NULL	0	NULL	statement 1	Process		is independent of					Nyv1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_140_1_61_s_216	9425154	( B) Binding of Sec17p and Sec18p to the vacuole is independent of the Nyv1p and Vam3p.	bind
48404	4	961	7	NULL	NULL	0	NULL	statement 1	Process		is independent of					 Vam3p	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_140_1_61_s_216	9425154	( B) Binding of Sec17p and Sec18p to the vacuole is independent of the Nyv1p and Vam3p.	bind
48405	5	961	7	NULL	NULL	0	NULL	statement 2	Process		is independent of					Nyv1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_140_1_61_s_216	9425154	( B) Binding of Sec17p and Sec18p to the vacuole is independent of the Nyv1p and Vam3p.	bind
48406	6	961	7	NULL	NULL	0	NULL	statement 2	Process		is independent of					Vam3p	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_140_1_61_s_216	9425154	( B) Binding of Sec17p and Sec18p to the vacuole is independent of the Nyv1p and Vam3p.	bind
356	1	962	6	NULL	NULL	0	NULL	Ssk2	NULL		bind	NULL				Pbs2	NULL		RSD-I		NULL		0	NULL	NULL	NULL	gw60_embo_22_14_3624_s_120	12853477	( B) Binding of Ssk2 to Pbs2 RSD-I.	bind
48410	1	962	7	NULL	NULL	0	NULL	Ssk2	GP		bind					Pbs2	GP		RSD-I		NULL		NULL	NULL	NULL	NULL	gw60_embo_22_14_3624_s_120	12853477	( B) Binding of Ssk2 to Pbs2 RSD-I.	bind
357	1	963	6	NULL	NULL	0	NULL	sum1	NULL		bind	NULL				HML-E	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_15_1811_s_156	16077008	( B) Binding of Sum1 to  HML-E required the D element.	bind
358	2	963	6	10	NULL	0	NULL	Statement 1	NULL		requires	NULL					NULL			D element	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_15_1811_s_156	16077008	( B) Binding of Sum1 to  HML-E required the D element.	bind
48411	1	963	7	NULL	NULL	0	NULL	Sum1	GP		bind					HML-E	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_15_1811_s_156	16077008	( B) Binding of Sum1 to  HML-E required the D element.	bind
48412	2	963	7	NULL	NULL	0	NULL	statement 1	Process		requires									D element	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_15_1811_s_156	16077008	( B) Binding of Sum1 to  HML-E required the D element.	bind
359	1	964	6	10	NULL	0	NULL	Env	NULL	HIV	bind	NULL				CXCR4	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_8_2078_s_15	16886053	( B) Binding of the HIV envelope glycoprotein (Env) to CXCR4 activates cellular autophagy,  which then leads to both apoptotic and autophagic cell death.	bind
51450	2	964	6	10	NULL	0	NULL	Env	NULL		is	NULL				envelope glycoprotein	NULL				NULL		0	NULL	NULL	NULL	gw70_jclininvest_116_8_2078_s_15	16886053	( B) Binding of the HIV envelope glycoprotein (Env) to CXCR4 activates cellular autophagy,  which then leads to both apoptotic and autophagic cell death.	bind
51451	3	964	6	10	NULL	0	NULL	statement 1	NULL		activates	NULL				cellular autophagy	NULL				NULL		0	NULL	NULL	NULL	gw70_jclininvest_116_8_2078_s_15	16886053	( B) Binding of the HIV envelope glycoprotein (Env) to CXCR4 activates cellular autophagy,  which then leads to both apoptotic and autophagic cell death.	bind
51452	4	964	6	10	NULL	0	NULL	statement 3	NULL		leads to	NULL				apoptotic cell death	NULL				NULL		0	NULL	NULL	NULL	gw70_jclininvest_116_8_2078_s_15	16886053	( B) Binding of the HIV envelope glycoprotein (Env) to CXCR4 activates cellular autophagy,  which then leads to both apoptotic and autophagic cell death.	bind
51453	5	964	6	10	NULL	0	NULL	statement 3	NULL		leads to	NULL				autophagic cell death	NULL				NULL		0	NULL	NULL	NULL	gw70_jclininvest_116_8_2078_s_15	16886053	( B) Binding of the HIV envelope glycoprotein (Env) to CXCR4 activates cellular autophagy,  which then leads to both apoptotic and autophagic cell death.	bind
48413	1	964	7	NULL	NULL	0	NULL	Env	GP	HIV	bind					CXCR4	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_8_2078_s_15	16886053	( B) Binding of the HIV envelope glycoprotein (Env) to CXCR4 activates cellular autophagy,  which then leads to both apoptotic and autophagic cell death.	bind
48414	2	964	7	NULL	NULL	0	NULL	statement 1	Process		activates					cellular autophagy	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_8_2078_s_15	16886053	( B) Binding of the HIV envelope glycoprotein (Env) to CXCR4 activates cellular autophagy,  which then leads to both apoptotic and autophagic cell death.	bind
48415	3	964	7	NULL	NULL	0	NULL	statement 2	Process		leads to					apoptotic cell death	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_8_2078_s_15	16886053	( B) Binding of the HIV envelope glycoprotein (Env) to CXCR4 activates cellular autophagy,  which then leads to both apoptotic and autophagic cell death.	bind
48416	4	964	7	NULL	NULL	0	NULL	statement 2	Process		leads to					autophagic cell death	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_8_2078_s_15	16886053	( B) Binding of the HIV envelope glycoprotein (Env) to CXCR4 activates cellular autophagy,  which then leads to both apoptotic and autophagic cell death.	bind
48417	5	964	7	NULL	NULL	0	NULL	Env	GP		is					envelope glycoprotein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_8_2078_s_15	16886053	( B) Binding of the HIV envelope glycoprotein (Env) to CXCR4 activates cellular autophagy,  which then leads to both apoptotic and autophagic cell death.	bind
360	1	966	6	NULL	NULL	0	NULL	Rad9	NULL		bind	NULL		PCNA-like domain		Rad17	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_100_4_1633_s_146	12578958	( B) Binding of the PCNA-like domain of Rad9 to Rad17.	bind
48418	1	966	7	NULL	NULL	0	NULL	Rad9	GP		bind			PCNA-like domain		Rad17	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_4_1633_s_146	12578958	( B) Binding of the PCNA-like domain of Rad9 to Rad17.	bind
361	1	967	6	NULL	NULL	0	NULL	TM7C	NULL		bind	NULL				Meta II	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_22_12854_s_149	9789004	( B) Binding of TM7C to Meta II as shown by immunoblotting.	bind
48419	1	967	7	NULL	NULL	0	NULL	TM7C	GP		bind					Meta II	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_22_12854_s_149	9789004	( B) Binding of TM7C to Meta II as shown by immunoblotting.	bind
363	1	968	6	NULL	NULL	0	NULL	trastuzumab 	NULL		bind	NULL		Fc variant		FcgammaRIIIa	NULL	human	V158		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_11_4005_s_46	16537476	( B) Binding of trastuzumab Fc variants to human V158 ( Left) and F158 ( Right) FcgammaRIIIa ( n = 2).	bind
364	2	968	6	NULL	NULL	0	NULL	trastuzumab 	NULL		bind	NULL		Fc variant		FcgammaRIIIa	NULL	human	F158		NULL		0	NULL	NULL	NULL	gw70_pnas_103_11_4005_s_46	16537476	( B) Binding of trastuzumab Fc variants to human V158 ( Left) and F158 ( Right) FcgammaRIIIa ( n = 2).	bind
48420	1	968	7	NULL	NULL	0	NULL	trastuzumab	GP		bind			Fc variants		FcgammaRIIIa	GP	human	V158		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_11_4005_s_46	16537476	( B) Binding of trastuzumab Fc variants to human V158 ( Left) and F158 ( Right) FcgammaRIIIa ( n = 2).	bind
48421	2	968	7	NULL	NULL	0	NULL	trastuzumab 	GP		bind			Fc variants		FcgammaRIIIa	GP	human	F158		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_11_4005_s_46	16537476	( B) Binding of trastuzumab Fc variants to human V158 ( Left) and F158 ( Right) FcgammaRIIIa ( n = 2).	bind
366	1	969	6	10	NULL	0	NULL	tRNAfMet	NULL		binds to	NULL					NULL			P site in AUG initiator codon	NULL		NULL	NULL	NULL	NULL	gw60_science_278_5340_1093_s_37	9353184	( B) Binding of tRNAfMet to the AUG initiator codon in the P (and E) site directs binding of ASLs to the UUU codon in the A site.	bind
367	2	969	6	10	NULL	0	NULL	ASLs	NULL		binds to	NULL					NULL			A site in UUU codon	NULL		NULL	NULL	NULL	NULL	gw60_science_278_5340_1093_s_37	9353184	( B) Binding of tRNAfMet to the AUG initiator codon in the P (and E) site directs binding of ASLs to the UUU codon in the A site.	bind
368	3	969	6	NULL	NULL	0	NULL	Statement 1	NULL		directs	NULL				Statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_science_278_5340_1093_s_37	9353184	( B) Binding of tRNAfMet to the AUG initiator codon in the P (and E) site directs binding of ASLs to the UUU codon in the A site.	bind
51454	4	969	6	10	NULL	0	NULL	tRNAfMet	NULL		bind	NULL					NULL			E site in AUG initiator codon	NULL		0	NULL	NULL	NULL	gw60_science_278_5340_1093_s_37	9353184	( B) Binding of tRNAfMet to the AUG initiator codon in the P (and E) site directs binding of ASLs to the UUU codon in the A site.	bind
51455	5	969	6	10	NULL	0	NULL	statement 4	NULL		directs	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_science_278_5340_1093_s_37	9353184	( B) Binding of tRNAfMet to the AUG initiator codon in the P (and E) site directs binding of ASLs to the UUU codon in the A site.	bind
48422	1	969	7	NULL	NULL	0	NULL	tRNAfMet	GP		bind									P site in AUG initiator codon	NULL		NULL	NULL	NULL	NULL	gw60_science_278_5340_1093_s_37	9353184	( B) Binding of tRNAfMet to the AUG initiator codon in the P (and E) site directs binding of ASLs to the UUU codon in the A site.	bind
48423	2	969	7	NULL	NULL	0	NULL	ASLs	GP		bind									A site in UUU codon	NULL		NULL	NULL	NULL	NULL	gw60_science_278_5340_1093_s_37	9353184	( B) Binding of tRNAfMet to the AUG initiator codon in the P (and E) site directs binding of ASLs to the UUU codon in the A site.	bind
48424	3	969	7	NULL	NULL	0	NULL	statement 1	Process		directs					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_278_5340_1093_s_37	9353184	( B) Binding of tRNAfMet to the AUG initiator codon in the P (and E) site directs binding of ASLs to the UUU codon in the A site.	bind
51456	4	969	7	NULL	NULL	0	NULL	tRNAfMet	GP		bind									E site in AUG initiator codon	NULL		NULL	NULL	NULL	NULL	gw60_science_278_5340_1093_s_37	9353184	( B) Binding of tRNAfMet to the AUG initiator codon in the P (and E) site directs binding of ASLs to the UUU codon in the A site.	bind
51457	5	969	7	NULL	NULL	0	NULL	statement 4	Process		directs					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_278_5340_1093_s_37	9353184	( B) Binding of tRNAfMet to the AUG initiator codon in the P (and E) site directs binding of ASLs to the UUU codon in the A site.	bind
371	1	970	6	10	NULL	0	NULL	vezatin	NULL		bind	NULL				myosin VIIA	NULL		tail		NULL	co-transfected HEK293 cells	NULL	NULL	NULL	NULL	gw60_embo_19_22_6020_s_63	11080149	( B) Binding of vezatin to the myosin VIIA tail in co-transfected HEK293 cells.	bind
48425	1	970	7	NULL	NULL	0	NULL	vezatin 	GP		bind					myosin VIIA 	GP		tail		NULL	co-transfected HEK293 cells	NULL	NULL	NULL	NULL	gw60_embo_19_22_6020_s_63	11080149	( B) Binding of vezatin to the myosin VIIA tail in co-transfected HEK293 cells.	bind
372	1	971	6	10	NULL	0	NULL	XIAP 	NULL		bind	NULL		H467A		MURR1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_1_244_s_177	14685266	( B) Binding of XIAP H467A to MURR1 and the effects of proteasome inhibition: 293 cells  were transfected as indicated and 1 day later half of the cultures were treated with  lactacystin (10 muM) for an additional 6 h.	bind
48439	1	971	7	NULL	NULL	0	NULL	XIAP	GP		bind			H467A		MURR1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_1_244_s_177	14685266	( B) Binding of XIAP H467A to MURR1 and the effects of proteasome inhibition: 293 cells  were transfected as indicated and 1 day later half of the cultures were treated with  lactacystin (10 muM) for an additional 6 h.	bind
373	1	972	6	NULL	NULL	0	NULL	YopN	NULL		bind	NULL				TyeA	NULL				NULL	Y.enterocolitica	0	NULL	NULL	NULL	gw60_embo_17_7_1907_s_172	9524114	( B) Binding of YopN with TyeA in  Y.enterocolitica.	bind
48440	1	972	7	NULL	NULL	0	NULL	YopN	GP		bind					TyeA	GP				NULL	Y.enterocolitica	NULL	NULL	NULL	NULL	gw60_embo_17_7_1907_s_172	9524114	( B) Binding of YopN with TyeA in  Y.enterocolitica.	bind
374	1	973	6	NULL	NULL	0	NULL	PIR-B peptides	NULL	phosphorylated	bind	NULL				GST-SHP1	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_5_2446_s_142	9482905	( B) Binding potential of phosphorylated PIR-B peptides to the GST-SHP 1.	bind
48441	1	973	7	NULL	NULL	0	NULL	PIR-B peptides	GP	phosphorylated	bind					GST-SHP1	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_5_2446_s_142	9482905	( B) Binding potential of phosphorylated PIR-B peptides to the GST-SHP 1.	bind
455	1	975	6	10	NULL	0	NULL	VPS4A protein	NULL	wild type	bind	NULL		1 - 84		GST-CHMP1B	NULL				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_39_13813_s_161	16174732	( B) Biosensor binding isotherms showing wild-type (WT) and L64A mutant VPS4A1 - 84 proteins binding GST-CHMP1B and GST-CHMP1B65 - 196.	bind
456	2	975	6	10	NULL	0	NULL	VPS4A protein	NULL	mutant	bind	NULL		L64A;;1 - 84		GST-CHMP1B	NULL				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_39_13813_s_161	16174732	( B) Biosensor binding isotherms showing wild-type (WT) and L64A mutant VPS4A1 - 84 proteins binding GST-CHMP1B and GST-CHMP1B65 - 196.	bind
457	3	975	6	10	NULL	0	NULL	VPS4A protein	NULL	wild type	bind	NULL		1 - 84		GST-CHMP1B	NULL		65 - 196		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_39_13813_s_161	16174732	( B) Biosensor binding isotherms showing wild-type (WT) and L64A mutant VPS4A1 - 84 proteins binding GST-CHMP1B and GST-CHMP1B65 - 196.	bind
458	4	975	6	10	NULL	0	NULL	VPS4A protein	NULL	mutant	bind	NULL		L64A;;1 - 84		GST-CHMP1B	NULL		65 - 196		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_39_13813_s_161	16174732	( B) Biosensor binding isotherms showing wild-type (WT) and L64A mutant VPS4A1 - 84 proteins binding GST-CHMP1B and GST-CHMP1B65 - 196.	bind
48442	1	975	7	NULL	NULL	0	NULL	VPS4A protein	GP	wild-type	bind			1-84		GST-CHMP1B	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_39_13813_s_161	16174732	( B) Biosensor binding isotherms showing wild-type (WT) and L64A mutant VPS4A1 - 84 proteins binding GST-CHMP1B and GST-CHMP1B65 - 196.	bind
48443	2	975	7	NULL	NULL	0	NULL	VPS4A protein	GP	mutant	bind			L64A;;1 - 84		GST-CHMP1B	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_39_13813_s_161	16174732	( B) Biosensor binding isotherms showing wild-type (WT) and L64A mutant VPS4A1 - 84 proteins binding GST-CHMP1B and GST-CHMP1B65 - 196.	bind
48444	3	975	7	NULL	NULL	0	NULL	VPS4A protein	GP	wild-type	bind			1-84		GST-CHMP1B	GP		65 - 196		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_39_13813_s_161	16174732	( B) Biosensor binding isotherms showing wild-type (WT) and L64A mutant VPS4A1 - 84 proteins binding GST-CHMP1B and GST-CHMP1B65 - 196.	bind
48445	4	975	7	NULL	NULL	0	NULL	VPS4A protein	GP	mutant	bind			L64A;;1 - 84		GST-CHMP1B	GP		65 - 196		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_39_13813_s_161	16174732	( B) Biosensor binding isotherms showing wild-type (WT) and L64A mutant VPS4A1 - 84 proteins binding GST-CHMP1B and GST-CHMP1B65 - 196.	bind
48446	5	975	7	NULL	NULL	0	NULL	WT	Organism		is					wild-type	Organism				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_39_13813_s_161	16174732	( B) Biosensor binding isotherms showing wild-type (WT) and L64A mutant VPS4A1 - 84 proteins binding GST-CHMP1B and GST-CHMP1B65 - 196.	bind
503	1	976	6	NULL	NULL	0	NULL	protein	NULL	lamprey	bind	NULL				GST-amphSH3 	NULL				NULL		0	NULL	NULL	NULL	gw60_science_276_5310_259_s_75	9092476	( B) Blots with dynamin antiserum DG1 on lamprey proteins bound to GST-amphSH3 (lane 1), GST-amphSH3mut (lane 2) (lanes 1 and 2 run in parallel), GST-amphSH3 (lane 3), and GST-amphSH3 in the presence of 300 muM of dynamin peptide (lane 4) (lanes 3 and 4 run in parallel) ( 24).	bind
504	2	976	6	NULL	NULL	0	NULL	protein	NULL	lamprey	bind	NULL				GST-amphSH3mut	NULL				NULL		0	NULL	NULL	NULL	gw60_science_276_5310_259_s_75	9092476	( B) Blots with dynamin antiserum DG1 on lamprey proteins bound to GST-amphSH3 (lane 1), GST-amphSH3mut (lane 2) (lanes 1 and 2 run in parallel), GST-amphSH3 (lane 3), and GST-amphSH3 in the presence of 300 muM of dynamin peptide (lane 4) (lanes 3 and 4 run in parallel) ( 24).	bind
613	3	976	6	NULL	NULL	0	NULL	Statement 1	NULL		in presence of	NULL				dynamin peptide	NULL				NULL		0	NULL	NULL	NULL	gw60_science_276_5310_259_s_75	9092476	( B) Blots with dynamin antiserum DG1 on lamprey proteins bound to GST-amphSH3 (lane 1), GST-amphSH3mut (lane 2) (lanes 1 and 2 run in parallel), GST-amphSH3 (lane 3), and GST-amphSH3 in the presence of 300 muM of dynamin peptide (lane 4) (lanes 3 and 4 run in parallel) ( 24).	bind
614	4	976	6	NULL	NULL	0	NULL	Statement 2	NULL		in presence of	NULL				dynamin peptide	NULL				NULL		0	NULL	NULL	NULL	gw60_science_276_5310_259_s_75	9092476	( B) Blots with dynamin antiserum DG1 on lamprey proteins bound to GST-amphSH3 (lane 1), GST-amphSH3mut (lane 2) (lanes 1 and 2 run in parallel), GST-amphSH3 (lane 3), and GST-amphSH3 in the presence of 300 muM of dynamin peptide (lane 4) (lanes 3 and 4 run in parallel) ( 24).	bind
48447	1	976	7	NULL	NULL	0	NULL	proteins	GP	lamprey	bind					 GST-amphSH3	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_276_5310_259_s_75	9092476	( B) Blots with dynamin antiserum DG1 on lamprey proteins bound to GST-amphSH3 (lane 1), GST-amphSH3mut (lane 2) (lanes 1 and 2 run in parallel), GST-amphSH3 (lane 3), and GST-amphSH3 in the presence of 300 muM of dynamin peptide (lane 4) (lanes 3 and 4 run in parallel) ( 24).	bind
48448	2	976	7	NULL	NULL	0	NULL	proteins	GP	lamprey	bind					 GST-amphSH3mut 	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_276_5310_259_s_75	9092476	( B) Blots with dynamin antiserum DG1 on lamprey proteins bound to GST-amphSH3 (lane 1), GST-amphSH3mut (lane 2) (lanes 1 and 2 run in parallel), GST-amphSH3 (lane 3), and GST-amphSH3 in the presence of 300 muM of dynamin peptide (lane 4) (lanes 3 and 4 run in parallel) ( 24).	bind
48449	3	976	7	NULL	NULL	0	NULL	statement 1	Process		in presence of					dynamin peptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_276_5310_259_s_75	9092476	( B) Blots with dynamin antiserum DG1 on lamprey proteins bound to GST-amphSH3 (lane 1), GST-amphSH3mut (lane 2) (lanes 1 and 2 run in parallel), GST-amphSH3 (lane 3), and GST-amphSH3 in the presence of 300 muM of dynamin peptide (lane 4) (lanes 3 and 4 run in parallel) ( 24).	bind
48450	4	976	7	NULL	NULL	0	NULL	statement 2	Process		in presence of					dynamin peptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_276_5310_259_s_75	9092476	( B) Blots with dynamin antiserum DG1 on lamprey proteins bound to GST-amphSH3 (lane 1), GST-amphSH3mut (lane 2) (lanes 1 and 2 run in parallel), GST-amphSH3 (lane 3), and GST-amphSH3 in the presence of 300 muM of dynamin peptide (lane 4) (lanes 3 and 4 run in parallel) ( 24).	bind
459	1	977	6	NULL	NULL	0	NULL	BLyS	NULL		bind	NULL				U-937 cells	NULL				NULL		0	NULL	NULL	NULL	gw60_science_285_5425_260_s_63	10398604	( B) BLyS binding to U-937 and the myeloma line IM-9.	bind
460	2	977	6	10	NULL	0	NULL	BLyS	NULL		bind	NULL				IM-9	NULL				NULL		NULL	NULL	NULL	NULL	gw60_science_285_5425_260_s_63	10398604	( B) BLyS binding to U-937 and the myeloma line IM-9.	bind
51458	3	977	6	10	NULL	0	NULL	IM-9	NULL		is a type of	NULL				myeloma line	NULL				NULL		0	NULL	NULL	NULL	gw60_science_285_5425_260_s_63	10398604	( B) BLyS binding to U-937 and the myeloma line IM-9.	bind
48451	1	977	7	NULL	NULL	0	NULL	BLyS	GP		bind					U-937	Cell				NULL		NULL	NULL	NULL	NULL	gw60_science_285_5425_260_s_63	10398604	( B) BLyS binding to U-937 and the myeloma line IM-9.	bind
48452	2	977	7	NULL	NULL	0	NULL	BLyS	GP		bind					IM-9	Cell				NULL		NULL	NULL	NULL	NULL	gw60_science_285_5425_260_s_63	10398604	( B) BLyS binding to U-937 and the myeloma line IM-9.	bind
48453	3	977	7	NULL	NULL	0	NULL	IM-9	Cell		is a type of					myeloma line	Cell				NULL		NULL	NULL	NULL	NULL	gw60_science_285_5425_260_s_63	10398604	( B) BLyS binding to U-937 and the myeloma line IM-9.	bind
461	1	978	6	NULL	NULL	0	NULL	BMP-6	NULL		bind	NULL				sclerostin	NULL	human			NULL		0	NULL	NULL	NULL	gw70_embo_22_23_6267_s_34	14633986	( B) BMP-6 binding to human sclerostin (circles) or a BSA-blocked plate (triangles) in  an ELISA-based association assay.	bind
48454	1	978	7	NULL	NULL	0	NULL	 BMP-6	GP		bind					sclerostin	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_embo_22_23_6267_s_34	14633986	( B) BMP-6 binding to human sclerostin (circles) or a BSA-blocked plate (triangles) in  an ELISA-based association assay.	bind
463	1	979	6	NULL	NULL	0	NULL	bis-ANS	NULL		bind	NULL				PAI-2	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_22_8_1753_s_136	12682008	( B) Calculated rate of  bis-ANS binding to PAI-2 (mean value of three experiments).	bind
48455	1	979	7	NULL	NULL	0	NULL	bis-ANS	Chemical		bind					PAI-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_8_1753_s_136	12682008	( B) Calculated rate of  bis-ANS binding to PAI-2 (mean value of three experiments).	bind
464	1	980	6	NULL	NULL	0	NULL	CARM1	NULL		bind	NULL	directly			p65	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_24_1_85_s_98	15616592	( B) CARM1 directly binds to p65.	bind
48456	1	980	7	NULL	NULL	0	NULL	 CARM1	GP		bind		directly			p65	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_1_85_s_98	15616592	( B) CARM1 directly binds to p65.	bind
465	1	981	6	NULL	NULL	0	NULL	Cd+2	NULL		bind	NULL				double cysteine channel	NULL	mutant			NULL	closed state	0	NULL	NULL	NULL	gw70_embo_23_24_4717_s_81	15565171	( B) Cd2+ binds R362C A419C double cysteine mutant channel in the closed state.	bind
48457	1	981	7	10	NULL	0	NULL	Cd2+	Chemical		bind					channel	CellComponent	double cysteine mutant	 R362C;; A419C		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_24_4717_s_81	15565171	( B) Cd2+ binds R362C A419C double cysteine mutant channel in the closed state.	bind
48458	2	981	7	NULL	NULL	0	NULL	statement 1	Process		occur in the 					channel	CellComponent	closed state of			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_24_4717_s_81	15565171	( B) Cd2+ binds R362C A419C double cysteine mutant channel in the closed state.	bind
466	1	982	6	NULL	NULL	0	NULL	CENP-B proteins	NULL		bind	NULL					NULL		CENP-B-box motifs		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_2_309_s_220	9548711	( b) CENP-B  proteins ( red circles) bind to  CENP-B-box motifs and undergo dimerization to cross-link the array into a more stable higher order configuration.	bind
51468	2	982	6	10	NULL	0	NULL	statement 1	NULL		undergo	NULL				dimerization	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_141_2_309_s_220	9548711	( b) CENP-B  proteins ( red circles) bind to  CENP-B-box motifs and undergo dimerization to cross-link the array into a more stable higher order configuration.	bind
51469	3	982	6	10	NULL	0	NULL	statement 2	NULL		crosslink	NULL				array	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_141_2_309_s_220	9548711	( b) CENP-B  proteins ( red circles) bind to  CENP-B-box motifs and undergo dimerization to cross-link the array into a more stable higher order configuration.	bind
51470	4	982	6	10	NULL	0	NULL	statement 3	NULL		leads to	NULL				configuration	NULL	stable;;higher order			NULL		0	NULL	NULL	NULL	gw60_cellbiol_141_2_309_s_220	9548711	( b) CENP-B  proteins ( red circles) bind to  CENP-B-box motifs and undergo dimerization to cross-link the array into a more stable higher order configuration.	bind
48459	1	982	7	NULL	NULL	0	NULL	CENP-B proteins	GP		bind								CENP-B-box motifs		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_2_309_s_220	9548711	( b) CENP-B  proteins ( red circles) bind to  CENP-B-box motifs and undergo dimerization to cross-link the array into a more stable higher order configuration.	bind
48460	2	982	7	NULL	NULL	0	NULL	statement 1	Process		undergo					dimerization	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_2_309_s_220	9548711	( b) CENP-B  proteins ( red circles) bind to  CENP-B-box motifs and undergo dimerization to cross-link the array into a more stable higher order configuration.	bind
48461	3	982	7	NULL	NULL	0	NULL	statement 2	Process		crosslink					array	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_2_309_s_220	9548711	( b) CENP-B  proteins ( red circles) bind to  CENP-B-box motifs and undergo dimerization to cross-link the array into a more stable higher order configuration.	bind
48462	4	982	7	NULL	NULL	0	NULL	statement 3	Process		leads to					configuration	Process	stable;;higher order			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_2_309_s_220	9548711	( b) CENP-B  proteins ( red circles) bind to  CENP-B-box motifs and undergo dimerization to cross-link the array into a more stable higher order configuration.	bind
51471	1	983	6	10	NULL	0	NULL	RalGDS	NULL	WT	bind	NULL		RBD		Ras	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_101_25_9223_s_186	15197281	( b) Changes in free enthalpy (deltadeltaH degrees ) plotted versus changes in entropy (TdeltadeltaS degrees )of binding between WT and mutant RalGDS-RBD/Ras.	bind
51472	2	983	6	10	NULL	0	NULL	RalGDS	NULL	mutant	bind	NULL		RBD		Ras	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_101_25_9223_s_186	15197281	( b) Changes in free enthalpy (deltadeltaH degrees ) plotted versus changes in entropy (TdeltadeltaS degrees )of binding between WT and mutant RalGDS-RBD/Ras.	bind
48463	1	983	7	NULL	NULL	0	NULL	RalGDS	GP	WT	bind			RBD		Ras	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_25_9223_s_186	15197281	( b) Changes in free enthalpy (deltadeltaH degrees ) plotted versus changes in entropy (TdeltadeltaS degrees )of binding between WT and mutant RalGDS-RBD/Ras.	bind
48464	2	983	7	NULL	NULL	0	NULL	RalGDS	GP	mutant	bind			RBD		Ras	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_25_9223_s_186	15197281	( b) Changes in free enthalpy (deltadeltaH degrees ) plotted versus changes in entropy (TdeltadeltaS degrees )of binding between WT and mutant RalGDS-RBD/Ras.	bind
468	1	985	6	NULL	NULL	0	NULL	E2F1	NULL		bind	NULL				E2F8	NULL			Promoter	NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_17_5458_s_190	16179649	( B) ChIP analysis of E2F1, E2F4 and E2F7 binding to the  E2F8 promoter.	bind
469	2	985	6	NULL	NULL	0	NULL	E2F4	NULL		bind	NULL				E2F8	NULL			Promoter	NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_17_5458_s_190	16179649	( B) ChIP analysis of E2F1, E2F4 and E2F7 binding to the  E2F8 promoter.	bind
470	3	985	6	NULL	NULL	0	NULL	E2f7	NULL		bind	NULL				E2f8	NULL			Promoter	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_17_5458_s_190	16179649	( B) ChIP analysis of E2F1, E2F4 and E2F7 binding to the  E2F8 promoter.	bind
48465	1	985	7	NULL	NULL	0	NULL	E2F1	GP		bind					E2F8	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_17_5458_s_190	16179649	( B) ChIP analysis of E2F1, E2F4 and E2F7 binding to the  E2F8 promoter.	bind
48466	2	985	7	NULL	NULL	0	NULL	 E2F4	GP		bind					E2F8	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_17_5458_s_190	16179649	( B) ChIP analysis of E2F1, E2F4 and E2F7 binding to the  E2F8 promoter.	bind
48467	3	985	7	NULL	NULL	0	NULL	 E2F7	GP		bind					 E2F8	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_17_5458_s_190	16179649	( B) ChIP analysis of E2F1, E2F4 and E2F7 binding to the  E2F8 promoter.	bind
471	1	986	6	NULL	NULL	0	NULL	Ino2-myc	NULL		bind	NULL				INO1	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_embo_24_9_1717_s_91	15861138	( B) ChIP analysis of Ino2-myc or Ino4-myc binding to the  INO1 promoter or the  HSP26 promoter (which served as a negative control).	bind
472	2	986	6	NULL	NULL	0	NULL	Ino4-myc	NULL		bind	NULL				INO1	NULL			Promoter	NULL		0	NULL	NULL	NULL	gw70_embo_24_9_1717_s_91	15861138	( B) ChIP analysis of Ino2-myc or Ino4-myc binding to the  INO1 promoter or the  HSP26 promoter (which served as a negative control).	bind
48468	1	986	7	NULL	NULL	0	NULL	Ino2-myc	GP		bind					INO1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_91	15861138	( B) ChIP analysis of Ino2-myc or Ino4-myc binding to the  INO1 promoter or the  HSP26 promoter (which served as a negative control).	bind
48469	2	986	7	NULL	NULL	0	NULL	Ino4-myc	GP		bind					 INO1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_91	15861138	( B) ChIP analysis of Ino2-myc or Ino4-myc binding to the  INO1 promoter or the  HSP26 promoter (which served as a negative control).	bind
48470	3	986	7	NULL	NULL	0	NULL	Ino2-myc	GP		bind					HSP26 	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_91	15861138	( B) ChIP analysis of Ino2-myc or Ino4-myc binding to the  INO1 promoter or the  HSP26 promoter (which served as a negative control).	bind
48471	4	986	7	NULL	NULL	0	NULL	Ino4-myc	GP		bind					HSP26	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_91	15861138	( B) ChIP analysis of Ino2-myc or Ino4-myc binding to the  INO1 promoter or the  HSP26 promoter (which served as a negative control).	bind
473	1	987	6	NULL	NULL	0	NULL	TFIIB	NULL		bind	NULL				Xist	NULL			P1 promoter	NULL	Ma1L and Ma2L	NULL	NULL	NULL	NULL	gw70_genesdev_19_12_1474_s_159	15964997	( B) ChIP analysis of TFIIB binding to the  Xist P1 and P2 promoters and the  Tsix promoter in Ma1L and Ma2L.	bind
474	2	987	6	NULL	NULL	0	NULL	TFIIB	NULL		bind	NULL				Xist	NULL			P2 promoter	NULL	Ma1L and Ma2L	NULL	NULL	NULL	NULL	gw70_genesdev_19_12_1474_s_159	15964997	( B) ChIP analysis of TFIIB binding to the  Xist P1 and P2 promoters and the  Tsix promoter in Ma1L and Ma2L.	bind
475	3	987	6	NULL	NULL	0	NULL	TFIIB	NULL		bind	NULL				Tsix	NULL			Promoter	NULL	Ma1L and Ma2L	0	NULL	NULL	NULL	gw70_genesdev_19_12_1474_s_159	15964997	( B) ChIP analysis of TFIIB binding to the  Xist P1 and P2 promoters and the  Tsix promoter in Ma1L and Ma2L.	bind
48472	1	987	7	NULL	NULL	0	NULL	TFIIB	GP		bind					 Xist	GP			P1 promoter	NULL	Ma1L and Ma2L	NULL	NULL	NULL	NULL	gw70_genesdev_19_12_1474_s_159	15964997	( B) ChIP analysis of TFIIB binding to the  Xist P1 and P2 promoters and the  Tsix promoter in Ma1L and Ma2L.	bind
48473	2	987	7	NULL	NULL	0	NULL	TFIIB	GP		bind					Xist	GP			P2 promoter	NULL	Ma1L and Ma2L	NULL	NULL	NULL	NULL	gw70_genesdev_19_12_1474_s_159	15964997	( B) ChIP analysis of TFIIB binding to the  Xist P1 and P2 promoters and the  Tsix promoter in Ma1L and Ma2L.	bind
48474	3	987	7	NULL	NULL	0	NULL	TFIIB	GP		bind					Tsix	GP			promoter	NULL	Ma1L and Ma2L	NULL	NULL	NULL	NULL	gw70_genesdev_19_12_1474_s_159	15964997	( B) ChIP analysis of TFIIB binding to the  Xist P1 and P2 promoters and the  Tsix promoter in Ma1L and Ma2L.	bind
476	1	988	6	NULL	NULL	0	NULL	Swi/nf	NULL		bind	NULL				GAL1	NULL			Promoter	NULL		0	NULL	NULL	NULL	gw70_embo_23_20_4040_s_72	15385957	( B) ChIP analysis of the binding of Swi/nf to the  GAL1 and  GAL7 promoters.	bind
477	2	988	6	NULL	NULL	0	NULL	Swi/nf	NULL		bind	NULL				GAL7	NULL			Promoter	NULL		0	NULL	NULL	NULL	gw70_embo_23_20_4040_s_72	15385957	( B) ChIP analysis of the binding of Swi/nf to the  GAL1 and  GAL7 promoters.	bind
48476	1	988	7	NULL	NULL	0	NULL	Swi/nf	GP		bind					GAL1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_embo_23_20_4040_s_72	15385957	( B) ChIP analysis of the binding of Swi/nf to the  GAL1 and  GAL7 promoters.	bind
48477	2	988	7	NULL	NULL	0	NULL	Swi/nf 	GP		bind					GAL7	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_embo_23_20_4040_s_72	15385957	( B) ChIP analysis of the binding of Swi/nf to the  GAL1 and  GAL7 promoters.	bind
478	1	989	6	10	NULL	0	NULL	Swi/nf	NULL		bind	NULL				GAL1 UASG 	NULL				NULL	yeast cells expressing Gal4-Gal11	NULL	NULL	NULL	NULL	gw70_embo_23_20_4040_s_148	15385957	( B) ChIP analysis of the binding of Swi/nf to the  GAL1 UASG in yeast cells expressing Gal4-Gal11.	bind
48478	1	989	7	NULL	NULL	0	NULL	Swi/nf	GP		bind					GAL1 UASG	GP				NULL	yeast cells expressing Gal4-Gal11	NULL	NULL	NULL	NULL	gw70_embo_23_20_4040_s_148	15385957	( B) ChIP analysis of the binding of Swi/nf to the  GAL1 UASG in yeast cells expressing Gal4-Gal11.	bind
479	1	991	6	NULL	NULL	0	NULL	MYC	NULL		bind	NULL				WRN	NULL			Promoter elements	NULL	in vivo	0	NULL	NULL	NULL	gw60_genesdev_17_13_1569_s_57	12842909	( B) ChIP detects  MYC binding to  WRN promoter elements in vivo.	bind
48479	1	991	7	NULL	NULL	0	NULL	MYC	GP		bind					WRN	GP			promoter elements	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_genesdev_17_13_1569_s_57	12842909	( B) ChIP detects  MYC binding to  WRN promoter elements in vivo.	bind
480	1	993	6	10	NULL	0	NULL	TBP	NULL		bind	NULL				INO1	NULL			Promoter	NULL	WT cells	NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_113	15861138	( B) ChIP was performed to determine the level of TBP bound to the  INO1 promoter in wild-type (WT) or  mot1-42 cells.	bind
481	2	993	6	NULL	NULL	0	NULL	TBP	NULL		bind	NULL				INO1	NULL			Promoter	NULL	mot1-42 cells	0	NULL	NULL	NULL	gw70_embo_24_9_1717_s_113	15861138	( B) ChIP was performed to determine the level of TBP bound to the  INO1 promoter in wild-type (WT) or  mot1-42 cells.	bind
51473	3	993	6	10	NULL	0	NULL	WT	NULL		is	NULL				wild-type	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_24_9_1717_s_113	15861138	( B) ChIP was performed to determine the level of TBP bound to the  INO1 promoter in wild-type (WT) or  mot1-42 cells.	bind
48480	1	993	7	NULL	NULL	0	NULL	TBP	GP		bind					INO1	GP			promoter	NULL	WT cells	NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_113	15861138	( B) ChIP was performed to determine the level of TBP bound to the  INO1 promoter in wild-type (WT) or  mot1-42 cells.	bind
48481	2	993	7	NULL	NULL	0	NULL	TBP	GP		bind					INO1	GP			promoter	NULL	mot1-42 cells	NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_113	15861138	( B) ChIP was performed to determine the level of TBP bound to the  INO1 promoter in wild-type (WT) or  mot1-42 cells.	bind
48482	3	993	7	NULL	NULL	0	NULL	WT	Organism		is					wild-type	Organism				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_113	15861138	( B) ChIP was performed to determine the level of TBP bound to the  INO1 promoter in wild-type (WT) or  mot1-42 cells.	bind
482	1	994	6	10	NULL	0	NULL	Mll	NULL		bind	NULL				p27Kip1	NULL			coding region	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_3_749_s_158	15640349	( B) ChIP with anti-MLLC antibody quantitated with Real-Time PCR shows that Mll binding to the  p27Kip1 coding region is much higher in cells expressing menin.	bind
483	2	994	6	10	NULL	0	NULL	Statement 1	NULL		is higher in	NULL				cells expressing menin 	NULL				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_3_749_s_158	15640349	( B) ChIP with anti-MLLC antibody quantitated with Real-Time PCR shows that Mll binding to the  p27Kip1 coding region is much higher in cells expressing menin.	bind
48483	1	994	7	NULL	NULL	0	NULL	Mll	GP		bind					p27Kip1	GP			coding region	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_3_749_s_158	15640349	( B) ChIP with anti-MLLC antibody quantitated with Real-Time PCR shows that Mll binding to the  p27Kip1 coding region is much higher in cells expressing menin.	bind
48484	3	994	7	10	NULL	0	NULL	statement 1	Process		is higher in					cells expressing menin	Cell				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_3_749_s_158	15640349	( B) ChIP with anti-MLLC antibody quantitated with Real-Time PCR shows that Mll binding to the  p27Kip1 coding region is much higher in cells expressing menin.	bind
484	1	995	6	NULL	NULL	0	NULL	Cholesterol	NULL		bind	NULL				Nef	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_100_14_8460_s_239	12824470	( b) Cholesterol  binding to Nef increases HIV infectivity.	bind
485	2	995	6	10	NULL	0	NULL	Statement 1	NULL		increases	NULL				HIV	NULL	infectivity of 			NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_14_8460_s_239	12824470	( b) Cholesterol  binding to Nef increases HIV infectivity.	bind
48485	1	995	7	NULL	NULL	0	NULL	Cholesterol	Chemical		bind					Nef	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_14_8460_s_239	12824470	( b) Cholesterol  binding to Nef increases HIV infectivity.	bind
48486	2	995	7	NULL	NULL	0	NULL	statement 1	Process		increases					HIV	Organism	infectivity of 			NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_14_8460_s_239	12824470	( b) Cholesterol  binding to Nef increases HIV infectivity.	bind
486	1	996	6	10	NULL	0	NULL	Gal4p-myc	NULL		bind	NULL				MTH1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_48_17302_s_158	16301536	( B) Chromatin IP showing galactose-specific binding of Gal4p-myc to  MTH1,  CIN5, and  GAL10 ( Left) and of Mth1p-myc to  HXT7	bind
487	2	996	6	10	NULL	0	NULL	Gal4p-myc	NULL		bind	NULL				CIN5	NULL				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_48_17302_s_158	16301536	( B) Chromatin IP showing galactose-specific binding of Gal4p-myc to  MTH1,  CIN5, and  GAL10 ( Left) and of Mth1p-myc to  HXT7	bind
488	3	996	6	10	NULL	0	NULL	Gal4p-myc	NULL		bind	NULL				GAL10	NULL				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_48_17302_s_158	16301536	( B) Chromatin IP showing galactose-specific binding of Gal4p-myc to  MTH1,  CIN5, and  GAL10 ( Left) and of Mth1p-myc to  HXT7	bind
489	4	996	6	NULL	NULL	0	NULL	Mth1p-myc	NULL		bind	NULL				HXT7	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_48_17302_s_158	16301536	( B) Chromatin IP showing galactose-specific binding of Gal4p-myc to  MTH1,  CIN5, and  GAL10 ( Left) and of Mth1p-myc to  HXT7	bind
51474	5	996	6	10	NULL	0	NULL	statement 1	NULL		is specific to	NULL				galactose	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_48_17302_s_158	16301536	( B) Chromatin IP showing galactose-specific binding of Gal4p-myc to  MTH1,  CIN5, and  GAL10 ( Left) and of Mth1p-myc to  HXT7	bind
51475	6	996	6	10	NULL	0	NULL	statement 2	NULL		is specific to	NULL				galactose	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_48_17302_s_158	16301536	( B) Chromatin IP showing galactose-specific binding of Gal4p-myc to  MTH1,  CIN5, and  GAL10 ( Left) and of Mth1p-myc to  HXT7	bind
51476	7	996	6	10	NULL	0	NULL	statement 3	NULL		is specific to	NULL				galactose	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_48_17302_s_158	16301536	( B) Chromatin IP showing galactose-specific binding of Gal4p-myc to  MTH1,  CIN5, and  GAL10 ( Left) and of Mth1p-myc to  HXT7	bind
48487	1	996	7	NULL	NULL	0	NULL	Gal4p-myc	GP		bind					MTH1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_48_17302_s_158	16301536	( B) Chromatin IP showing galactose-specific binding of Gal4p-myc to  MTH1,  CIN5, and  GAL10 ( Left) and of Mth1p-myc to  HXT7	bind
48488	2	996	7	NULL	NULL	0	NULL	Gal4p-myc	GP		 bind					CIN5	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_48_17302_s_158	16301536	( B) Chromatin IP showing galactose-specific binding of Gal4p-myc to  MTH1,  CIN5, and  GAL10 ( Left) and of Mth1p-myc to  HXT7	bind
48489	3	996	7	NULL	NULL	0	NULL	Gal4p-myc	GP		bind					GAL10	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_48_17302_s_158	16301536	( B) Chromatin IP showing galactose-specific binding of Gal4p-myc to  MTH1,  CIN5, and  GAL10 ( Left) and of Mth1p-myc to  HXT7	bind
48490	4	996	7	NULL	NULL	0	NULL	 Mth1p-myc	GP		bind					HXT7	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_48_17302_s_158	16301536	( B) Chromatin IP showing galactose-specific binding of Gal4p-myc to  MTH1,  CIN5, and  GAL10 ( Left) and of Mth1p-myc to  HXT7	bind
48491	5	996	7	NULL	NULL	0	NULL	statement 1	Process		is specific to					galactose	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_48_17302_s_158	16301536	( B) Chromatin IP showing galactose-specific binding of Gal4p-myc to  MTH1,  CIN5, and  GAL10 ( Left) and of Mth1p-myc to  HXT7	bind
48492	6	996	7	NULL	NULL	0	NULL	statement 2	Process		is specific to					galactose	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_48_17302_s_158	16301536	( B) Chromatin IP showing galactose-specific binding of Gal4p-myc to  MTH1,  CIN5, and  GAL10 ( Left) and of Mth1p-myc to  HXT7	bind
48493	7	996	7	NULL	NULL	0	NULL	statement 3	Process		is specific to					galactose	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_48_17302_s_158	16301536	( B) Chromatin IP showing galactose-specific binding of Gal4p-myc to  MTH1,  CIN5, and  GAL10 ( Left) and of Mth1p-myc to  HXT7	bind
490	1	997	6	NULL	NULL	0	NULL	DLX2	NULL		bind	NULL				Dlx5/6	NULL			intergenic enhancer	NULL	neonatal retina in situ	0	NULL	NULL	NULL	gw70_nucleicacidsres_32_3_884_s_161	14769946	( b) Chromatin IP: DLX2 but not DLX1 binds to the  Dlx5/6 intergenic enhancer in neonatal retina  in situ. ChIP was performed using P0 retina and specific DLX1 or DLX2 antibodies.	bind
491	2	997	6	NULL	NULL	0	NULL	Dlx1	NULL		does not bind	NULL				Dlx5/6	NULL			intergenic enhancer	NULL	neonatal retina in situ	0	NULL	NULL	NULL	gw70_nucleicacidsres_32_3_884_s_161	14769946	( b) Chromatin IP: DLX2 but not DLX1 binds to the  Dlx5/6 intergenic enhancer in neonatal retina  in situ. ChIP was performed using P0 retina and specific DLX1 or DLX2 antibodies.	bind
48494	1	997	7	NULL	NULL	0	NULL	DLX2	GP		bind					Dlx5/6	GP	 		intergenic enhancer	NULL	neonatal retina in situ	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_32_3_884_s_161	14769946	( b) Chromatin IP: DLX2 but not DLX1 binds to the  Dlx5/6 intergenic enhancer in neonatal retina  in situ. ChIP was performed using P0 retina and specific DLX1 or DLX2 antibodies.	bind
48495	2	997	7	NULL	NULL	0	NULL	DLX1	GP		does not bind					Dlx5/6 	GP	 		intergenic enhancer	NULL	neonatal retina in situ	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_32_3_884_s_161	14769946	( b) Chromatin IP: DLX2 but not DLX1 binds to the  Dlx5/6 intergenic enhancer in neonatal retina  in situ. ChIP was performed using P0 retina and specific DLX1 or DLX2 antibodies.	bind
492	1	998	6	NULL	NULL	0	NULL	Chs5p	NULL		bind	NULL				Arf1p	NULL	activated			NULL		0	NULL	NULL	NULL	gw70_embo_25_5_943_s_128	16498409	( B) Chs5p binds to activated Arf1p.	bind
48496	1	998	7	NULL	NULL	0	NULL	Chs5p	GP		bind					Arf1p	GP	activated			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_5_943_s_128	16498409	( B) Chs5p binds to activated Arf1p.	bind
493	1	999	6	NULL	NULL	0	NULL	CIITA	NULL		bind	NULL				GTP	NULL				NULL		0	NULL	NULL	NULL	gw60_science_285_5432_1402_s_50	10464099	( B) CIITA binds GTP.	bind
48497	1	999	7	NULL	NULL	0	NULL	CIITA	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_285_5432_1402_s_50	10464099	( B) CIITA binds GTP.	bind
494	1	1002	6	NULL	NULL	0	NULL	TRAF2	NULL		bind	NULL				CD40 fragment	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_19_10395_s_92	10984535	( B) Close-up view of the CD40 fragment bound to TRAF2 and TRAF3.	bind
495	2	1002	6	NULL	NULL	0	NULL	traf3	NULL		bind	NULL				CD40 fragment	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_19_10395_s_92	10984535	( B) Close-up view of the CD40 fragment bound to TRAF2 and TRAF3.	bind
48498	1	1002	7	NULL	NULL	0	NULL	CD40 fragment 	GP		bind					TRAF2	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_19_10395_s_92	10984535	( B) Close-up view of the CD40 fragment bound to TRAF2 and TRAF3.	bind
48499	2	1002	7	NULL	NULL	0	NULL	CD40 fragment 	GP		bind					TRAF3	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_19_10395_s_92	10984535	( B) Close-up view of the CD40 fragment bound to TRAF2 and TRAF3.	bind
496	2	1005	6	10	NULL	0	NULL	CHO cells	NULL		express	NULL				alphaIIbbeta3	NULL	WT;;human			NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_39	12730600	( B) Comparison of constitutive and DTT-induced fibrinogen binding to CHO cells expressing wild-type (WT) human alphaIIbbeta3 or G708N beta3 mutant.	bind
497	3	1005	6	10	NULL	0	NULL	CHO cells	NULL		express	NULL				beta3	NULL	mutant	G708N		NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_39	12730600	( B) Comparison of constitutive and DTT-induced fibrinogen binding to CHO cells expressing wild-type (WT) human alphaIIbbeta3 or G708N beta3 mutant.	bind
51477	1	1005	6	10	NULL	0	NULL	fibrinogen	NULL		is induced by	NULL				DTT	NULL				NULL		0	NULL	NULL	NULL	gw60_science_300_5620_795_s_39	12730600	( B) Comparison of constitutive and DTT-induced fibrinogen binding to CHO cells expressing wild-type (WT) human alphaIIbbeta3 or G708N beta3 mutant.	bind
51478	4	1005	6	10	NULL	0	NULL	fibrinogen	NULL	constitutive	bind	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_science_300_5620_795_s_39	12730600	( B) Comparison of constitutive and DTT-induced fibrinogen binding to CHO cells expressing wild-type (WT) human alphaIIbbeta3 or G708N beta3 mutant.	bind
51479	5	1005	6	10	NULL	0	NULL	fibrinogen	NULL	constitutive	bind	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_science_300_5620_795_s_39	12730600	( B) Comparison of constitutive and DTT-induced fibrinogen binding to CHO cells expressing wild-type (WT) human alphaIIbbeta3 or G708N beta3 mutant.	bind
51480	6	1005	6	10	NULL	0	NULL	statement 4	NULL		is an alternative to	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_science_300_5620_795_s_39	12730600	( B) Comparison of constitutive and DTT-induced fibrinogen binding to CHO cells expressing wild-type (WT) human alphaIIbbeta3 or G708N beta3 mutant.	bind
51481	7	1005	6	10	NULL	0	NULL	statement 1	NULL		bind	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_science_300_5620_795_s_39	12730600	( B) Comparison of constitutive and DTT-induced fibrinogen binding to CHO cells expressing wild-type (WT) human alphaIIbbeta3 or G708N beta3 mutant.	bind
51482	8	1005	6	10	NULL	0	NULL	statement 1	NULL		bind	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_science_300_5620_795_s_39	12730600	( B) Comparison of constitutive and DTT-induced fibrinogen binding to CHO cells expressing wild-type (WT) human alphaIIbbeta3 or G708N beta3 mutant.	bind
51483	9	1005	6	10	NULL	0	NULL	statement 7	NULL		is an alternative to	NULL				statement 8	NULL				NULL		0	NULL	NULL	NULL	gw60_science_300_5620_795_s_39	12730600	( B) Comparison of constitutive and DTT-induced fibrinogen binding to CHO cells expressing wild-type (WT) human alphaIIbbeta3 or G708N beta3 mutant.	bind
48500	1	1005	7	NULL	NULL	0	NULL	CHO cells	Cell		express					 alphaIIbbeta3	GP	WT;; human			NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_39	12730600	( B) Comparison of constitutive and DTT-induced fibrinogen binding to CHO cells expressing wild-type (WT) human alphaIIbbeta3 or G708N beta3 mutant.	bind
48501	2	1005	7	NULL	NULL	0	NULL	CHO cells	Cell		express					 beta3	GP	mutant	G708N		NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_39	12730600	( B) Comparison of constitutive and DTT-induced fibrinogen binding to CHO cells expressing wild-type (WT) human alphaIIbbeta3 or G708N beta3 mutant.	bind
48502	3	1005	7	NULL	NULL	0	NULL	fibrinogen	GP	Constitutive	bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_39	12730600	( B) Comparison of constitutive and DTT-induced fibrinogen binding to CHO cells expressing wild-type (WT) human alphaIIbbeta3 or G708N beta3 mutant.	bind
48503	4	1005	7	NULL	NULL	0	NULL	fibrinogen	GP	Constitutive	bind					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_39	12730600	( B) Comparison of constitutive and DTT-induced fibrinogen binding to CHO cells expressing wild-type (WT) human alphaIIbbeta3 or G708N beta3 mutant.	bind
48504	5	1005	7	NULL	NULL	0	NULL	DTT	Chemical		induce					fibrinogen	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_39	12730600	( B) Comparison of constitutive and DTT-induced fibrinogen binding to CHO cells expressing wild-type (WT) human alphaIIbbeta3 or G708N beta3 mutant.	bind
48505	6	1005	7	NULL	NULL	0	NULL	statement 5	GP		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_39	12730600	( B) Comparison of constitutive and DTT-induced fibrinogen binding to CHO cells expressing wild-type (WT) human alphaIIbbeta3 or G708N beta3 mutant.	bind
48506	7	1005	7	NULL	NULL	0	NULL	statement 5	GP		bind					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_39	12730600	( B) Comparison of constitutive and DTT-induced fibrinogen binding to CHO cells expressing wild-type (WT) human alphaIIbbeta3 or G708N beta3 mutant.	bind
51484	8	1005	7	NULL	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_39	12730600	( B) Comparison of constitutive and DTT-induced fibrinogen binding to CHO cells expressing wild-type (WT) human alphaIIbbeta3 or G708N beta3 mutant.	bind
51485	9	1005	7	NULL	NULL	0	NULL	statement 6	Process		is an alternative to					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_39	12730600	( B) Comparison of constitutive and DTT-induced fibrinogen binding to CHO cells expressing wild-type (WT) human alphaIIbbeta3 or G708N beta3 mutant.	bind
498	1	1006	6	NULL	NULL	0	NULL	RecA	NULL		bind	NULL				lambda-EMBL3	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_21_12295_s_155	9770480	( B) Comparison of RecA binding kinetics to lambda-EMBL3, lambda-EMBL3 dimer, and 156Gmac for a constant externally applied force of 45 pN.	bind
499	2	1006	6	NULL	NULL	0	NULL	RecA	NULL		bind	NULL				lambda-EMBL3 dimer	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_21_12295_s_155	9770480	( B) Comparison of RecA binding kinetics to lambda-EMBL3, lambda-EMBL3 dimer, and 156Gmac for a constant externally applied force of 45 pN.	bind
500	3	1006	6	NULL	NULL	0	NULL	RecA	NULL		bind	NULL				156Gmac	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_21_12295_s_155	9770480	( B) Comparison of RecA binding kinetics to lambda-EMBL3, lambda-EMBL3 dimer, and 156Gmac for a constant externally applied force of 45 pN.	bind
48507	1	1006	7	NULL	NULL	0	NULL	RecA	GP		bind					lambda-EMBL3	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_21_12295_s_155	9770480	( B) Comparison of RecA binding kinetics to lambda-EMBL3, lambda-EMBL3 dimer, and 156Gmac for a constant externally applied force of 45 pN.	bind
48508	2	1006	7	NULL	NULL	0	NULL	RecA	GP		bind					lambda-EMBL3 dimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_21_12295_s_155	9770480	( B) Comparison of RecA binding kinetics to lambda-EMBL3, lambda-EMBL3 dimer, and 156Gmac for a constant externally applied force of 45 pN.	bind
48509	3	1006	7	NULL	NULL	0	NULL	RecA	GP		bind					156Gmac	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_21_12295_s_155	9770480	( B) Comparison of RecA binding kinetics to lambda-EMBL3, lambda-EMBL3 dimer, and 156Gmac for a constant externally applied force of 45 pN.	bind
501	1	1007	6	10	NULL	0	NULL	CBF-A	NULL		bind	NULL					NULL	rat		HRE	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_19_3762_s_203	11000268	( B) Comparison of the binding affinity of CBF-A to the rat HRE and CArG box.	bind
502	2	1007	6	10	NULL	0	NULL	CBF-A	NULL		bind	NULL					NULL	rat		CArG box	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_19_3762_s_203	11000268	( B) Comparison of the binding affinity of CBF-A to the rat HRE and CArG box.	bind
48510	1	1007	7	NULL	NULL	0	NULL	CBF-A	GP		bind							rat		HRE	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_19_3762_s_203	11000268	( B) Comparison of the binding affinity of CBF-A to the rat HRE and CArG box.	bind
48511	2	1007	7	NULL	NULL	0	NULL	CBF-A	GP		bind							rat		CArG box	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_19_3762_s_203	11000268	( B) Comparison of the binding affinity of CBF-A to the rat HRE and CArG box.	bind
615	1	1013	6	NULL	NULL	0	NULL	ORF80	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_4973_s_225	11812827	( B) Competition experiments with 250 nM ORF80 bound to 5 nM DNA.	bind
48512	1	1013	7	NULL	NULL	0	NULL	ORF80	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_4973_s_225	11812827	( B) Competition experiments with 250 nM ORF80 bound to 5 nM DNA.	bind
653	1	1014	6	10	NULL	0	NULL	SRC1	NULL		bind	NULL				cyclin D1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_22_3488_s_145	9832502	( B) Competition of cyclin D1-SRC1 binding by SRC1 peptides.	bind
654	2	1014	6	10	NULL	0	NULL	SRC1 peptide	NULL		bind	NULL				cyclin D1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_22_3488_s_145	9832502	( B) Competition of cyclin D1-SRC1 binding by SRC1 peptides.	bind
51486	3	1014	6	10	NULL	0	NULL	statement 2	NULL		competes with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_22_3488_s_145	9832502	( B) Competition of cyclin D1-SRC1 binding by SRC1 peptides.	bind
48513	1	1014	7	NULL	NULL	0	NULL	SRC1	GP		bind					cyclin D1	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_22_3488_s_145	9832502	( B) Competition of cyclin D1-SRC1 binding by SRC1 peptides.	bind
48514	2	1014	7	NULL	NULL	0	NULL	SRC1 peptides	GP		bind					cyclin D1	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_22_3488_s_145	9832502	( B) Competition of cyclin D1-SRC1 binding by SRC1 peptides.	bind
48515	3	1014	7	NULL	NULL	0	NULL	statement 2	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_22_3488_s_145	9832502	( B) Competition of cyclin D1-SRC1 binding by SRC1 peptides.	bind
655	1	1015	6	10	NULL	0	NULL	Prz	NULL		bind	NULL				E-HRP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_158	11027358	( B) Competition of E-HRP binding by the alpha1-adrenergic ligand prazosin (Prz), alpha2-adrenergic ligands yohimbine (Yh) and clonidine (Cln), beta-adrenergic ligand propranolol (Pro), and the dopamine D2 receptor ligand quinpirole (Quin).	bind
656	2	1015	6	10	NULL	0	NULL	Prz	NULL		is	NULL				prazosin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_158	11027358	( B) Competition of E-HRP binding by the alpha1-adrenergic ligand prazosin (Prz), alpha2-adrenergic ligands yohimbine (Yh) and clonidine (Cln), beta-adrenergic ligand propranolol (Pro), and the dopamine D2 receptor ligand quinpirole (Quin).	bind
657	3	1015	6	10	NULL	0	NULL	Yh	NULL		bind	NULL				E-HRP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_158	11027358	( B) Competition of E-HRP binding by the alpha1-adrenergic ligand prazosin (Prz), alpha2-adrenergic ligands yohimbine (Yh) and clonidine (Cln), beta-adrenergic ligand propranolol (Pro), and the dopamine D2 receptor ligand quinpirole (Quin).	bind
658	4	1015	6	10	NULL	0	NULL	Yh	NULL		is	NULL				yohimbine	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_158	11027358	( B) Competition of E-HRP binding by the alpha1-adrenergic ligand prazosin (Prz), alpha2-adrenergic ligands yohimbine (Yh) and clonidine (Cln), beta-adrenergic ligand propranolol (Pro), and the dopamine D2 receptor ligand quinpirole (Quin).	bind
659	5	1015	6	10	NULL	0	NULL	Cln	NULL		bind	NULL				E-HRP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_158	11027358	( B) Competition of E-HRP binding by the alpha1-adrenergic ligand prazosin (Prz), alpha2-adrenergic ligands yohimbine (Yh) and clonidine (Cln), beta-adrenergic ligand propranolol (Pro), and the dopamine D2 receptor ligand quinpirole (Quin).	bind
660	6	1015	6	10	NULL	0	NULL	Cln	NULL		is 	NULL				clonidine	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_158	11027358	( B) Competition of E-HRP binding by the alpha1-adrenergic ligand prazosin (Prz), alpha2-adrenergic ligands yohimbine (Yh) and clonidine (Cln), beta-adrenergic ligand propranolol (Pro), and the dopamine D2 receptor ligand quinpirole (Quin).	bind
661	7	1015	6	NULL	NULL	0	NULL	beta-adrenergic ligand propranolol	NULL		bind	NULL				E-HRP	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_158	11027358	( B) Competition of E-HRP binding by the alpha1-adrenergic ligand prazosin (Prz), alpha2-adrenergic ligands yohimbine (Yh) and clonidine (Cln), beta-adrenergic ligand propranolol (Pro), and the dopamine D2 receptor ligand quinpirole (Quin).	bind
662	8	1015	6	NULL	NULL	0	NULL	Pro	NULL		is	NULL				beta-adrenergic ligand propranolol	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_158	11027358	( B) Competition of E-HRP binding by the alpha1-adrenergic ligand prazosin (Prz), alpha2-adrenergic ligands yohimbine (Yh) and clonidine (Cln), beta-adrenergic ligand propranolol (Pro), and the dopamine D2 receptor ligand quinpirole (Quin).	bind
663	9	1015	6	NULL	NULL	0	NULL	dopamine D2 receptor ligand quinpirole	NULL		bind	NULL				E-HRP	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_158	11027358	( B) Competition of E-HRP binding by the alpha1-adrenergic ligand prazosin (Prz), alpha2-adrenergic ligands yohimbine (Yh) and clonidine (Cln), beta-adrenergic ligand propranolol (Pro), and the dopamine D2 receptor ligand quinpirole (Quin).	bind
664	10	1015	6	NULL	NULL	0	NULL	Quin	NULL		is	NULL				dopamine D2 receptor ligand quinpirole	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_158	11027358	( B) Competition of E-HRP binding by the alpha1-adrenergic ligand prazosin (Prz), alpha2-adrenergic ligands yohimbine (Yh) and clonidine (Cln), beta-adrenergic ligand propranolol (Pro), and the dopamine D2 receptor ligand quinpirole (Quin).	bind
48516	1	1015	7	NULL	NULL	0	NULL	Prz	Chemical		bind					E-HRP	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_158	11027358	( B) Competition of E-HRP binding by the alpha1-adrenergic ligand prazosin (Prz), alpha2-adrenergic ligands yohimbine (Yh) and clonidine (Cln), beta-adrenergic ligand propranolol (Pro), and the dopamine D2 receptor ligand quinpirole (Quin).	bind
48517	2	1015	7	NULL	NULL	0	NULL	Yh	Chemical		bind					E-HRP	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_158	11027358	( B) Competition of E-HRP binding by the alpha1-adrenergic ligand prazosin (Prz), alpha2-adrenergic ligands yohimbine (Yh) and clonidine (Cln), beta-adrenergic ligand propranolol (Pro), and the dopamine D2 receptor ligand quinpirole (Quin).	bind
48518	3	1015	7	NULL	NULL	0	NULL	Cln	Chemical		bind					E-HRP	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_158	11027358	( B) Competition of E-HRP binding by the alpha1-adrenergic ligand prazosin (Prz), alpha2-adrenergic ligands yohimbine (Yh) and clonidine (Cln), beta-adrenergic ligand propranolol (Pro), and the dopamine D2 receptor ligand quinpirole (Quin).	bind
48519	4	1015	7	NULL	NULL	0	NULL	Pro	Chemical		bind					E-HRP	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_158	11027358	( B) Competition of E-HRP binding by the alpha1-adrenergic ligand prazosin (Prz), alpha2-adrenergic ligands yohimbine (Yh) and clonidine (Cln), beta-adrenergic ligand propranolol (Pro), and the dopamine D2 receptor ligand quinpirole (Quin).	bind
48520	5	1015	7	NULL	NULL	0	NULL	Quin	Chemical		bind					E-HRP	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_158	11027358	( B) Competition of E-HRP binding by the alpha1-adrenergic ligand prazosin (Prz), alpha2-adrenergic ligands yohimbine (Yh) and clonidine (Cln), beta-adrenergic ligand propranolol (Pro), and the dopamine D2 receptor ligand quinpirole (Quin).	bind
48521	6	1015	7	NULL	NULL	0	NULL	Prz	Chemical		is					prazosin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_158	11027358	( B) Competition of E-HRP binding by the alpha1-adrenergic ligand prazosin (Prz), alpha2-adrenergic ligands yohimbine (Yh) and clonidine (Cln), beta-adrenergic ligand propranolol (Pro), and the dopamine D2 receptor ligand quinpirole (Quin).	bind
48522	7	1015	7	NULL	NULL	0	NULL	Prz	Chemical		is a type of					alpha1-adrenergic ligand	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_158	11027358	( B) Competition of E-HRP binding by the alpha1-adrenergic ligand prazosin (Prz), alpha2-adrenergic ligands yohimbine (Yh) and clonidine (Cln), beta-adrenergic ligand propranolol (Pro), and the dopamine D2 receptor ligand quinpirole (Quin).	bind
48523	8	1015	7	NULL	NULL	0	NULL	Yh	Chemical		is					 yohimbine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_158	11027358	( B) Competition of E-HRP binding by the alpha1-adrenergic ligand prazosin (Prz), alpha2-adrenergic ligands yohimbine (Yh) and clonidine (Cln), beta-adrenergic ligand propranolol (Pro), and the dopamine D2 receptor ligand quinpirole (Quin).	bind
48524	9	1015	7	NULL	NULL	0	NULL	Yh	Chemical		is a type of					alpha2-adrenergic ligand	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_158	11027358	( B) Competition of E-HRP binding by the alpha1-adrenergic ligand prazosin (Prz), alpha2-adrenergic ligands yohimbine (Yh) and clonidine (Cln), beta-adrenergic ligand propranolol (Pro), and the dopamine D2 receptor ligand quinpirole (Quin).	bind
48525	10	1015	7	NULL	NULL	0	NULL	Cln	Chemical		is					clonidine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_158	11027358	( B) Competition of E-HRP binding by the alpha1-adrenergic ligand prazosin (Prz), alpha2-adrenergic ligands yohimbine (Yh) and clonidine (Cln), beta-adrenergic ligand propranolol (Pro), and the dopamine D2 receptor ligand quinpirole (Quin).	bind
48526	11	1015	7	NULL	NULL	0	NULL	Cln	Chemical		is a type of					alpha2-adrenergic ligand	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_158	11027358	( B) Competition of E-HRP binding by the alpha1-adrenergic ligand prazosin (Prz), alpha2-adrenergic ligands yohimbine (Yh) and clonidine (Cln), beta-adrenergic ligand propranolol (Pro), and the dopamine D2 receptor ligand quinpirole (Quin).	bind
48527	12	1015	7	NULL	NULL	0	NULL	Pro	Chemical		is					propranolol	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_158	11027358	( B) Competition of E-HRP binding by the alpha1-adrenergic ligand prazosin (Prz), alpha2-adrenergic ligands yohimbine (Yh) and clonidine (Cln), beta-adrenergic ligand propranolol (Pro), and the dopamine D2 receptor ligand quinpirole (Quin).	bind
48528	13	1015	7	NULL	NULL	0	NULL	Pro	Chemical		is a type of					beta-adrenergic ligand	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_158	11027358	( B) Competition of E-HRP binding by the alpha1-adrenergic ligand prazosin (Prz), alpha2-adrenergic ligands yohimbine (Yh) and clonidine (Cln), beta-adrenergic ligand propranolol (Pro), and the dopamine D2 receptor ligand quinpirole (Quin).	bind
48529	14	1015	7	NULL	NULL	0	NULL	Quin	Chemical		is					quinpirole	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_158	11027358	( B) Competition of E-HRP binding by the alpha1-adrenergic ligand prazosin (Prz), alpha2-adrenergic ligands yohimbine (Yh) and clonidine (Cln), beta-adrenergic ligand propranolol (Pro), and the dopamine D2 receptor ligand quinpirole (Quin).	bind
48530	15	1015	7	NULL	NULL	0	NULL	Quin	Chemical		is a type of					dopamine D2 receptor ligand	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11603_s_158	11027358	( B) Competition of E-HRP binding by the alpha1-adrenergic ligand prazosin (Prz), alpha2-adrenergic ligands yohimbine (Yh) and clonidine (Cln), beta-adrenergic ligand propranolol (Pro), and the dopamine D2 receptor ligand quinpirole (Quin).	bind
665	1	1016	6	10	NULL	0	NULL	GST MBNL1	NULL		bind	NULL				cTNT MSE1 4 RNA	NULL	labeled;;chicken			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_15_3103_s_135	15257297	( B) Competition of GST MBNL1 binding to labeled chicken cTNT MSE1 4 RNA by nonlabeled  MSE RNAs.	bind
666	2	1016	6	10	NULL	0	NULL	GST MBNL1	NULL		bind	NULL				MSE RNAs	NULL	nonlabeled			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_15_3103_s_135	15257297	( B) Competition of GST MBNL1 binding to labeled chicken cTNT MSE1 4 RNA by nonlabeled  MSE RNAs.	bind
51487	3	1016	6	10	NULL	0	NULL	statement 2	NULL		competes with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_23_15_3103_s_135	15257297	( B) Competition of GST MBNL1 binding to labeled chicken cTNT MSE1 4 RNA by nonlabeled  MSE RNAs.	bind
48531	1	1016	7	NULL	NULL	0	NULL	GST MBNL1	GP		bind					cTNT MSE1 4 RNA	GP	labeled;;chicken			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_15_3103_s_135	15257297	( B) Competition of GST MBNL1 binding to labeled chicken cTNT MSE1 4 RNA by nonlabeled  MSE RNAs.	bind
48532	2	1016	7	NULL	NULL	0	NULL	GST MBNL1	GP		bind					MSE RNA	GP	nonlabeled			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_15_3103_s_135	15257297	( B) Competition of GST MBNL1 binding to labeled chicken cTNT MSE1 4 RNA by nonlabeled  MSE RNAs.	bind
48533	3	1016	7	NULL	NULL	0	NULL	statement 2	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_15_3103_s_135	15257297	( B) Competition of GST MBNL1 binding to labeled chicken cTNT MSE1 4 RNA by nonlabeled  MSE RNAs.	bind
667	1	1017	6	NULL	NULL	0	NULL	PIF3 	NULL		bind	NULL				G-wt	NULL				NULL		0	NULL	NULL	NULL	gw60_science_288_5467_859_s_96	10797009	( B) Competition of PIF3 binding to G-wt by the different G-box sequences from the four light-regulated genes.	bind
669	2	1017	6	10	NULL	0	NULL	PIF3	NULL		bind	NULL				light regulated genes	NULL			G-box sequences	NULL		NULL	NULL	NULL	NULL	gw60_science_288_5467_859_s_96	10797009	( B) Competition of PIF3 binding to G-wt by the different G-box sequences from the four light-regulated genes.	bind
51488	3	1017	6	10	NULL	0	NULL	statement 2	NULL		competes with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_science_288_5467_859_s_96	10797009	( B) Competition of PIF3 binding to G-wt by the different G-box sequences from the four light-regulated genes.	bind
48534	1	1017	7	NULL	NULL	0	NULL	PIF3	GP		bind					 G-wt	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_288_5467_859_s_96	10797009	( B) Competition of PIF3 binding to G-wt by the different G-box sequences from the four light-regulated genes.	bind
48535	2	1017	7	NULL	NULL	0	NULL	PIF3	GP		bind					light-regulated gene	GP			G-box sequences	NULL		NULL	NULL	NULL	NULL	gw60_science_288_5467_859_s_96	10797009	( B) Competition of PIF3 binding to G-wt by the different G-box sequences from the four light-regulated genes.	bind
48536	3	1017	7	NULL	NULL	0	NULL	statement 2	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_288_5467_859_s_96	10797009	( B) Competition of PIF3 binding to G-wt by the different G-box sequences from the four light-regulated genes.	bind
671	1	1018	6	NULL	NULL	0	NULL	HSV gD	NULL		bind	NULL				sV(HIgR)-Fc	NULL				NULL	In vitro	NULL	NULL	NULL	NULL	gw60_pnas_95_26_15700_s_174	9861033	( B) Competition of the  in vitro binding of HSV gD to sV(HIgR)-Fc by mAb R1.302 to PRR1 (R1.302,  ), mAb to gD HD1 (HD1,  ), or purified mouse IgGs (IgG, x).	bind
673	2	1018	6	NULL	NULL	0	NULL	Prr1	NULL		competes	NULL				Statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_26_15700_s_174	9861033	( B) Competition of the  in vitro binding of HSV gD to sV(HIgR)-Fc by mAb R1.302 to PRR1 (R1.302,  ), mAb to gD HD1 (HD1,  ), or purified mouse IgGs (IgG, x).	bind
674	3	1018	6	NULL	NULL	0	NULL	gD HD1	NULL		competes	NULL				Statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_26_15700_s_174	9861033	( B) Competition of the  in vitro binding of HSV gD to sV(HIgR)-Fc by mAb R1.302 to PRR1 (R1.302,  ), mAb to gD HD1 (HD1,  ), or purified mouse IgGs (IgG, x).	bind
675	4	1018	6	NULL	NULL	0	NULL	IgGs	NULL	purified mouse	competes	NULL				Statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_26_15700_s_174	9861033	( B) Competition of the  in vitro binding of HSV gD to sV(HIgR)-Fc by mAb R1.302 to PRR1 (R1.302,  ), mAb to gD HD1 (HD1,  ), or purified mouse IgGs (IgG, x).	bind
48537	1	1018	7	NULL	NULL	0	NULL	 HSV gD	GP		bind					sV(HIgR)-Fc	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_pnas_95_26_15700_s_174	9861033	( B) Competition of the  in vitro binding of HSV gD to sV(HIgR)-Fc by mAb R1.302 to PRR1 (R1.302,  ), mAb to gD HD1 (HD1,  ), or purified mouse IgGs (IgG, x).	bind
48538	2	1018	7	NULL	NULL	0	NULL	HSV gD	GP		bind					mAb R1.302	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_26_15700_s_174	9861033	( B) Competition of the  in vitro binding of HSV gD to sV(HIgR)-Fc by mAb R1.302 to PRR1 (R1.302,  ), mAb to gD HD1 (HD1,  ), or purified mouse IgGs (IgG, x).	bind
48539	3	1018	7	NULL	NULL	0	NULL	HSV gD 	GP		bind					PRR1	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_26_15700_s_174	9861033	( B) Competition of the  in vitro binding of HSV gD to sV(HIgR)-Fc by mAb R1.302 to PRR1 (R1.302,  ), mAb to gD HD1 (HD1,  ), or purified mouse IgGs (IgG, x).	bind
48540	4	1018	7	NULL	NULL	0	NULL	statement 2	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_26_15700_s_174	9861033	( B) Competition of the  in vitro binding of HSV gD to sV(HIgR)-Fc by mAb R1.302 to PRR1 (R1.302,  ), mAb to gD HD1 (HD1,  ), or purified mouse IgGs (IgG, x).	bind
48541	5	1018	7	NULL	NULL	0	NULL	statement 3	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_26_15700_s_174	9861033	( B) Competition of the  in vitro binding of HSV gD to sV(HIgR)-Fc by mAb R1.302 to PRR1 (R1.302,  ), mAb to gD HD1 (HD1,  ), or purified mouse IgGs (IgG, x).	bind
48652	6	1018	7	NULL	NULL	0	NULL	HSV gD	GP		bind					gD HD1 mAb	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_26_15700_s_174	9861033	( B) Competition of the  in vitro binding of HSV gD to sV(HIgR)-Fc by mAb R1.302 to PRR1 (R1.302,  ), mAb to gD HD1 (HD1,  ), or purified mouse IgGs (IgG, x).	bind
48653	7	1018	7	NULL	NULL	0	NULL	HSV gD	GP		bind					IgG	GP	purified mouse			NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_26_15700_s_174	9861033	( B) Competition of the  in vitro binding of HSV gD to sV(HIgR)-Fc by mAb R1.302 to PRR1 (R1.302,  ), mAb to gD HD1 (HD1,  ), or purified mouse IgGs (IgG, x).	bind
48654	8	1018	7	NULL	NULL	0	NULL	statement 6	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_26_15700_s_174	9861033	( B) Competition of the  in vitro binding of HSV gD to sV(HIgR)-Fc by mAb R1.302 to PRR1 (R1.302,  ), mAb to gD HD1 (HD1,  ), or purified mouse IgGs (IgG, x).	bind
48655	9	1018	7	NULL	NULL	0	NULL	statement 7	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_26_15700_s_174	9861033	( B) Competition of the  in vitro binding of HSV gD to sV(HIgR)-Fc by mAb R1.302 to PRR1 (R1.302,  ), mAb to gD HD1 (HD1,  ), or purified mouse IgGs (IgG, x).	bind
676	1	1019	6	NULL	NULL	0	NULL	IAA	NULL		binds	NULL				Insulin	NULL	human	Tyr14A		NULL		0	NULL	NULL	NULL	gw70_jclininvest_114_4_589_s_128	15314696	( B) Competitive inhibition of IAA binding to Tyr14A [125] human insulin using human insulin (open circles), human B28lysB29pro insulin (open  triangles), human A13trpB28lysB29pro insulin (shaded squares), porcine insulin (shaded  circles), sheep A8his insulin (filled diamonds), and fish insulin (crosses).	bind
677	2	1019	6	NULL	NULL	0	NULL	Insulin	NULL	human	competes	NULL				Statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jclininvest_114_4_589_s_128	15314696	( B) Competitive inhibition of IAA binding to Tyr14A [125] human insulin using human insulin (open circles), human B28lysB29pro insulin (open  triangles), human A13trpB28lysB29pro insulin (shaded squares), porcine insulin (shaded  circles), sheep A8his insulin (filled diamonds), and fish insulin (crosses).	bind
678	3	1019	6	NULL	NULL	0	NULL	Insulin	NULL	human	competes	NULL		B28lysB29pro		Statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jclininvest_114_4_589_s_128	15314696	( B) Competitive inhibition of IAA binding to Tyr14A [125] human insulin using human insulin (open circles), human B28lysB29pro insulin (open  triangles), human A13trpB28lysB29pro insulin (shaded squares), porcine insulin (shaded  circles), sheep A8his insulin (filled diamonds), and fish insulin (crosses).	bind
679	4	1019	6	NULL	NULL	0	NULL	Insulin	NULL	human	competes	NULL		A13trpB28lysB29pro		Statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jclininvest_114_4_589_s_128	15314696	( B) Competitive inhibition of IAA binding to Tyr14A [125] human insulin using human insulin (open circles), human B28lysB29pro insulin (open  triangles), human A13trpB28lysB29pro insulin (shaded squares), porcine insulin (shaded  circles), sheep A8his insulin (filled diamonds), and fish insulin (crosses).	bind
680	5	1019	6	NULL	NULL	0	NULL	Insulin	NULL	porcine	competes	NULL				Statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jclininvest_114_4_589_s_128	15314696	( B) Competitive inhibition of IAA binding to Tyr14A [125] human insulin using human insulin (open circles), human B28lysB29pro insulin (open  triangles), human A13trpB28lysB29pro insulin (shaded squares), porcine insulin (shaded  circles), sheep A8his insulin (filled diamonds), and fish insulin (crosses).	bind
681	6	1019	6	NULL	NULL	0	NULL	Insulin	NULL	sheep	competes	NULL		A8his		Statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jclininvest_114_4_589_s_128	15314696	( B) Competitive inhibition of IAA binding to Tyr14A [125] human insulin using human insulin (open circles), human B28lysB29pro insulin (open  triangles), human A13trpB28lysB29pro insulin (shaded squares), porcine insulin (shaded  circles), sheep A8his insulin (filled diamonds), and fish insulin (crosses).	bind
683	7	1019	6	NULL	NULL	0	NULL	Insulin	NULL	fish	competes	NULL				Statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jclininvest_114_4_589_s_128	15314696	( B) Competitive inhibition of IAA binding to Tyr14A [125] human insulin using human insulin (open circles), human B28lysB29pro insulin (open  triangles), human A13trpB28lysB29pro insulin (shaded squares), porcine insulin (shaded  circles), sheep A8his insulin (filled diamonds), and fish insulin (crosses).	bind
48542	1	1019	7	NULL	NULL	0	NULL	IAA 	Chemical		bind					 insulin	GP	human	 Tyr14A		NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_4_589_s_128	15314696	( B) Competitive inhibition of IAA binding to Tyr14A [125] human insulin using human insulin (open circles), human B28lysB29pro insulin (open  triangles), human A13trpB28lysB29pro insulin (shaded squares), porcine insulin (shaded  circles), sheep A8his insulin (filled diamonds), and fish insulin (crosses).	bind
48543	2	1019	7	NULL	NULL	0	NULL	IAA	Chemical		bind					insulin	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_4_589_s_128	15314696	( B) Competitive inhibition of IAA binding to Tyr14A [125] human insulin using human insulin (open circles), human B28lysB29pro insulin (open  triangles), human A13trpB28lysB29pro insulin (shaded squares), porcine insulin (shaded  circles), sheep A8his insulin (filled diamonds), and fish insulin (crosses).	bind
48544	3	1019	7	NULL	NULL	0	NULL	IAA	Chemical		bind					proinsulin	GP	human	B28lysB29		NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_4_589_s_128	15314696	( B) Competitive inhibition of IAA binding to Tyr14A [125] human insulin using human insulin (open circles), human B28lysB29pro insulin (open  triangles), human A13trpB28lysB29pro insulin (shaded squares), porcine insulin (shaded  circles), sheep A8his insulin (filled diamonds), and fish insulin (crosses).	bind
48545	4	1019	7	NULL	NULL	0	NULL	IAA	Chemical		bind					pro insulin	GP	human	A13trpB28lysB29		NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_4_589_s_128	15314696	( B) Competitive inhibition of IAA binding to Tyr14A [125] human insulin using human insulin (open circles), human B28lysB29pro insulin (open  triangles), human A13trpB28lysB29pro insulin (shaded squares), porcine insulin (shaded  circles), sheep A8his insulin (filled diamonds), and fish insulin (crosses).	bind
48546	5	1019	7	NULL	NULL	0	NULL	IAA	Chemical		bind					insulin	GP	porcine			NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_4_589_s_128	15314696	( B) Competitive inhibition of IAA binding to Tyr14A [125] human insulin using human insulin (open circles), human B28lysB29pro insulin (open  triangles), human A13trpB28lysB29pro insulin (shaded squares), porcine insulin (shaded  circles), sheep A8his insulin (filled diamonds), and fish insulin (crosses).	bind
48547	6	1019	7	NULL	NULL	0	NULL	IAA	Chemical		bind					insulin	GP	sheep	 A8his		NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_4_589_s_128	15314696	( B) Competitive inhibition of IAA binding to Tyr14A [125] human insulin using human insulin (open circles), human B28lysB29pro insulin (open  triangles), human A13trpB28lysB29pro insulin (shaded squares), porcine insulin (shaded  circles), sheep A8his insulin (filled diamonds), and fish insulin (crosses).	bind
48548	7	1019	7	NULL	NULL	0	NULL	IAA	Chemical		bind					insulin	GP	fish			NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_4_589_s_128	15314696	( B) Competitive inhibition of IAA binding to Tyr14A [125] human insulin using human insulin (open circles), human B28lysB29pro insulin (open  triangles), human A13trpB28lysB29pro insulin (shaded squares), porcine insulin (shaded  circles), sheep A8his insulin (filled diamonds), and fish insulin (crosses).	bind
48575	8	1019	7	NULL	NULL	0	NULL	statement 2	Process		inhibit		competitively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_4_589_s_128	15314696	( B) Competitive inhibition of IAA binding to Tyr14A [125] human insulin using human insulin (open circles), human B28lysB29pro insulin (open  triangles), human A13trpB28lysB29pro insulin (shaded squares), porcine insulin (shaded  circles), sheep A8his insulin (filled diamonds), and fish insulin (crosses).	bind
48576	9	1019	7	NULL	NULL	0	NULL	statement 3	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_4_589_s_128	15314696	( B) Competitive inhibition of IAA binding to Tyr14A [125] human insulin using human insulin (open circles), human B28lysB29pro insulin (open  triangles), human A13trpB28lysB29pro insulin (shaded squares), porcine insulin (shaded  circles), sheep A8his insulin (filled diamonds), and fish insulin (crosses).	bind
48577	10	1019	7	NULL	NULL	0	NULL	statement 4	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_4_589_s_128	15314696	( B) Competitive inhibition of IAA binding to Tyr14A [125] human insulin using human insulin (open circles), human B28lysB29pro insulin (open  triangles), human A13trpB28lysB29pro insulin (shaded squares), porcine insulin (shaded  circles), sheep A8his insulin (filled diamonds), and fish insulin (crosses).	bind
48578	11	1019	7	NULL	NULL	0	NULL	statement 5	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_4_589_s_128	15314696	( B) Competitive inhibition of IAA binding to Tyr14A [125] human insulin using human insulin (open circles), human B28lysB29pro insulin (open  triangles), human A13trpB28lysB29pro insulin (shaded squares), porcine insulin (shaded  circles), sheep A8his insulin (filled diamonds), and fish insulin (crosses).	bind
48579	12	1019	7	NULL	NULL	0	NULL	statement 6	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_4_589_s_128	15314696	( B) Competitive inhibition of IAA binding to Tyr14A [125] human insulin using human insulin (open circles), human B28lysB29pro insulin (open  triangles), human A13trpB28lysB29pro insulin (shaded squares), porcine insulin (shaded  circles), sheep A8his insulin (filled diamonds), and fish insulin (crosses).	bind
48580	13	1019	7	NULL	NULL	0	NULL	statement 7	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_4_589_s_128	15314696	( B) Competitive inhibition of IAA binding to Tyr14A [125] human insulin using human insulin (open circles), human B28lysB29pro insulin (open  triangles), human A13trpB28lysB29pro insulin (shaded squares), porcine insulin (shaded  circles), sheep A8his insulin (filled diamonds), and fish insulin (crosses).	bind
684	2	1020	6	10	NULL	0	NULL	calstabin2	NULL	WT	bind	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_9_3456_s_129	16481613	( B) Concentration curve of WT calstabin2 vs. calstabin2 - D37V binding to PKA-phosphorylated  RyR2 showed that, at physiologic levels of calstabin2, calstabin2 - D37V exhibited  increased binding to PKA-phosphorylated RyR2 compared with WT calstabin2.	bind
685	3	1020	6	10	NULL	0	NULL	calstabin2 	NULL		bind	NULL		D37V		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_9_3456_s_129	16481613	( B) Concentration curve of WT calstabin2 vs. calstabin2 - D37V binding to PKA-phosphorylated  RyR2 showed that, at physiologic levels of calstabin2, calstabin2 - D37V exhibited  increased binding to PKA-phosphorylated RyR2 compared with WT calstabin2.	bind
51491	1	1020	6	10	NULL	0	NULL	RyR2	NULL		is phosphorylated by	NULL				PKA	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_103_9_3456_s_129	16481613	( B) Concentration curve of WT calstabin2 vs. calstabin2 - D37V binding to PKA-phosphorylated  RyR2 showed that, at physiologic levels of calstabin2, calstabin2 - D37V exhibited  increased binding to PKA-phosphorylated RyR2 compared with WT calstabin2.	bind
51492	4	1020	6	10	NULL	0	NULL	statement 3	NULL	affinity of	is higher than	NULL				statement 2	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw70_pnas_103_9_3456_s_129	16481613	( B) Concentration curve of WT calstabin2 vs. calstabin2 - D37V binding to PKA-phosphorylated  RyR2 showed that, at physiologic levels of calstabin2, calstabin2 - D37V exhibited  increased binding to PKA-phosphorylated RyR2 compared with WT calstabin2.	bind
48581	1	1020	7	NULL	NULL	0	NULL	RyR2	GP		is phosphorylated by					PKA	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_9_3456_s_129	16481613	( B) Concentration curve of WT calstabin2 vs. calstabin2 - D37V binding to PKA-phosphorylated  RyR2 showed that, at physiologic levels of calstabin2, calstabin2 - D37V exhibited  increased binding to PKA-phosphorylated RyR2 compared with WT calstabin2.	bind
48582	2	1020	7	NULL	NULL	0	NULL	calstabin2	Chemical		bind			D37V		statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_9_3456_s_129	16481613	( B) Concentration curve of WT calstabin2 vs. calstabin2 - D37V binding to PKA-phosphorylated  RyR2 showed that, at physiologic levels of calstabin2, calstabin2 - D37V exhibited  increased binding to PKA-phosphorylated RyR2 compared with WT calstabin2.	bind
48583	3	1020	7	NULL	NULL	0	NULL	calstabin2	Chemical	WT	bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_9_3456_s_129	16481613	( B) Concentration curve of WT calstabin2 vs. calstabin2 - D37V binding to PKA-phosphorylated  RyR2 showed that, at physiologic levels of calstabin2, calstabin2 - D37V exhibited  increased binding to PKA-phosphorylated RyR2 compared with WT calstabin2.	bind
48584	4	1020	7	NULL	NULL	0	NULL	statement 2	Process	affinity of	is higher than					statement 3	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_9_3456_s_129	16481613	( B) Concentration curve of WT calstabin2 vs. calstabin2 - D37V binding to PKA-phosphorylated  RyR2 showed that, at physiologic levels of calstabin2, calstabin2 - D37V exhibited  increased binding to PKA-phosphorylated RyR2 compared with WT calstabin2.	bind
686	1	1023	6	NULL	NULL	0	NULL	CPO	NULL		bind	NULL				CPO-BP	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_17_6195_s_134	15840715	( B) Correlation plot for inhibition of [3]CPO binding to CPO-BP and FP-rhodamine labeling of KIAA1363.	bind
48585	1	1023	7	NULL	NULL	0	NULL	CPO	Chemical		bind					CPO-BP	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_17_6195_s_134	15840715	( B) Correlation plot for inhibition of [3]CPO binding to CPO-BP and FP-rhodamine labeling of KIAA1363.	bind
688	1	1024	6	NULL	NULL	0	NULL	CRSP	NULL		bind	NULL				Ni2+-NTA-agarose resin	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_96_13_7137_s_80	10377381	( b) CRSP binds to Ni2+-NTA-agarose resin in the presence of competing imidazole.	bind
689	2	1024	6	NULL	NULL	0	NULL	Statement 1	NULL		occurs in presence of	NULL				imidazole	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_96_13_7137_s_80	10377381	( b) CRSP binds to Ni2+-NTA-agarose resin in the presence of competing imidazole.	bind
48586	1	1024	7	NULL	NULL	0	NULL	CRSP	GP		bind					Ni2+-NTA-agarose resin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_13_7137_s_80	10377381	( b) CRSP binds to Ni2+-NTA-agarose resin in the presence of competing imidazole.	bind
48587	2	1024	7	NULL	NULL	0	NULL	statement 1	Process		in presence of					imidazole	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_13_7137_s_80	10377381	( b) CRSP binds to Ni2+-NTA-agarose resin in the presence of competing imidazole.	bind
690	1	1025	6	10	NULL	0	NULL	Ctf18-Myc	NULL		does not bind	NULL	specifically			telomere VIR	NULL				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_7_1505_s_171	16525505	( B) Ctf18-Myc does not bind specifically to telomere VIR.	bind
48588	1	1025	7	NULL	NULL	0	NULL	Ctf18-Myc	GP		does not bind		specifically			telomere VIR	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_7_1505_s_171	16525505	( B) Ctf18-Myc does not bind specifically to telomere VIR.	bind
691	1	1026	6	NULL	NULL	0	NULL	Cubilin	NULL		bind	NULL				megalin	NULL				NULL	In vitro	NULL	NULL	NULL	NULL	gw70_annurevnutr_21_0_407_s_122	11375443	( b) Cubilin binds in vitro to megalin ( 59).	bind
48589	1	1026	7	NULL	NULL	0	NULL	Cubilin	GP		bind					megalin	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_annurevnutr_21_0_407_s_122	11375443	( b) Cubilin binds in vitro to megalin ( 59).	bind
692	1	1028	6	NULL	NULL	0	NULL	Cdc45	NULL		bind	NULL				chromatin	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_17_9_1141_s_145	12730133	( B) Cut5-dependent binding of Cdc45 and Sld5 to chromatin.	bind
693	2	1028	6	NULL	NULL	0	NULL	Sld5	NULL		bind	NULL				chromatin	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_17_9_1141_s_145	12730133	( B) Cut5-dependent binding of Cdc45 and Sld5 to chromatin.	bind
694	3	1028	6	NULL	NULL	0	NULL	Statement 1	NULL		is dependent on	NULL				Cut5	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_17_9_1141_s_145	12730133	( B) Cut5-dependent binding of Cdc45 and Sld5 to chromatin.	bind
695	4	1028	6	NULL	NULL	0	NULL	statement 2	NULL		is dependent on	NULL				Cut5	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_17_9_1141_s_145	12730133	( B) Cut5-dependent binding of Cdc45 and Sld5 to chromatin.	bind
48590	1	1028	7	NULL	NULL	0	NULL	Cdc45	GP		bind					chromatin	Chromosome				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_9_1141_s_145	12730133	( B) Cut5-dependent binding of Cdc45 and Sld5 to chromatin.	bind
48591	2	1028	7	NULL	NULL	0	NULL	Sld5	GP		bind					chromatin	Chromosome				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_9_1141_s_145	12730133	( B) Cut5-dependent binding of Cdc45 and Sld5 to chromatin.	bind
48592	3	1028	7	NULL	NULL	0	NULL	statement 1	Process		is dependent on					Cut5	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_9_1141_s_145	12730133	( B) Cut5-dependent binding of Cdc45 and Sld5 to chromatin.	bind
48593	4	1028	7	NULL	NULL	0	NULL	statement 2	Process		is dependent on					Cut5	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_9_1141_s_145	12730133	( B) Cut5-dependent binding of Cdc45 and Sld5 to chromatin.	bind
696	1	1029	6	10	NULL	0	NULL	GST-Cdc20p	NULL		bind	NULL				MBP-Hsl1p	NULL		667-872		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_18_2381_s_147	11562348	( B) D box-dependent binding of GST-Cdc20p to MBP-Hsl1p667-872.	bind
697	2	1029	6	NULL	NULL	0	NULL	Statement 1	NULL		is dependent on	NULL					NULL		D box		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_18_2381_s_147	11562348	( B) D box-dependent binding of GST-Cdc20p to MBP-Hsl1p667-872.	bind
48594	1	1029	7	NULL	NULL	0	NULL	GST-Cdc20p	GP		bind					MBP-Hsl1p	GP		667-872		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_18_2381_s_147	11562348	( B) D box-dependent binding of GST-Cdc20p to MBP-Hsl1p667-872.	bind
48595	2	1029	7	NULL	NULL	0	NULL	statement 1	Process		is dependent on									D-box	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_18_2381_s_147	11562348	( B) D box-dependent binding of GST-Cdc20p to MBP-Hsl1p667-872.	bind
698	1	1030	6	10	NULL	0	NULL	d4T triphosphate	NULL		bind	NULL					NULL	 variant	H122G		NULL		NULL	NULL	NULL	NULL	gw60_embo_19_14_3520_s_55	10899107	( B) d4T triphosphate bound to the H122G variant.	bind
48596	1	1030	7	NULL	NULL	0	NULL	d4T triphosphate	Chemical		bind							variant	H122G		NULL		NULL	NULL	NULL	NULL	gw60_embo_19_14_3520_s_55	10899107	( B) d4T triphosphate bound to the H122G variant.	bind
871	1	1032	6	NULL	NULL	0	NULL	Dectin-1	NULL		bind	NULL				S. cerevisiae	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_24_6_1277_s_70	15729357	( B) Dectin-1 binds  S. cerevisiae and  C. albicans equivalently.	bind
872	2	1032	6	NULL	NULL	0	NULL	Dectin-1	NULL		bind	NULL				C.albicans	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_24_6_1277_s_70	15729357	( B) Dectin-1 binds  S. cerevisiae and  C. albicans equivalently.	bind
51493	3	1032	6	10	NULL	0	NULL	statement 1	NULL	affinity of	is equivalent to	NULL				statement 2	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw70_embo_24_6_1277_s_70	15729357	( B) Dectin-1 binds  S. cerevisiae and  C. albicans equivalently.	bind
48597	1	1032	7	NULL	NULL	0	NULL	Dectin-1	GP		bind					S. cerevisiae	Organism				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_6_1277_s_70	15729357	( B) Dectin-1 binds  S. cerevisiae and  C. albicans equivalently.	bind
48598	2	1032	7	NULL	NULL	0	NULL	Dectin-1	GP		bind					C. albicans	Organism				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_6_1277_s_70	15729357	( B) Dectin-1 binds  S. cerevisiae and  C. albicans equivalently.	bind
48599	3	1032	7	NULL	NULL	0	NULL	statement 1	Process	affinity of	is equivalent to					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw70_embo_24_6_1277_s_70	15729357	( B) Dectin-1 binds  S. cerevisiae and  C. albicans equivalently.	bind
699	1	1033	6	NULL	NULL	0	NULL	JIP-1	NULL		bind	NULL				JNK1	NULL				NULL		0	NULL	NULL	NULL	gw60_science_281_5383_1671_s_80	9733513	( B) Deletion analysis of the binding of JIP-1 to JNK1, MKK7, MLK3, and DLK.	bind
700	2	1033	6	NULL	NULL	0	NULL	JIP-1	NULL		bind	NULL				MKK7	NULL				NULL		0	NULL	NULL	NULL	gw60_science_281_5383_1671_s_80	9733513	( B) Deletion analysis of the binding of JIP-1 to JNK1, MKK7, MLK3, and DLK.	bind
701	3	1033	6	NULL	NULL	0	NULL	JIP-1	NULL		bind	NULL				MLK3	NULL				NULL		0	NULL	NULL	NULL	gw60_science_281_5383_1671_s_80	9733513	( B) Deletion analysis of the binding of JIP-1 to JNK1, MKK7, MLK3, and DLK.	bind
702	4	1033	6	NULL	NULL	0	NULL	JIP-1	NULL		bind	NULL				DLK	NULL				NULL		0	NULL	NULL	NULL	gw60_science_281_5383_1671_s_80	9733513	( B) Deletion analysis of the binding of JIP-1 to JNK1, MKK7, MLK3, and DLK.	bind
48600	1	1033	7	NULL	NULL	0	NULL	JIP-1	GP		bind					JNK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5383_1671_s_80	9733513	( B) Deletion analysis of the binding of JIP-1 to JNK1, MKK7, MLK3, and DLK.	bind
48601	2	1033	7	NULL	NULL	0	NULL	JIP-1	GP		bind					MKK7	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5383_1671_s_80	9733513	( B) Deletion analysis of the binding of JIP-1 to JNK1, MKK7, MLK3, and DLK.	bind
48602	3	1033	7	NULL	NULL	0	NULL	JIP-1	GP		bind					MLK3	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5383_1671_s_80	9733513	( B) Deletion analysis of the binding of JIP-1 to JNK1, MKK7, MLK3, and DLK.	bind
48603	4	1033	7	NULL	NULL	0	NULL	JIP-1	GP		bind					DLK	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5383_1671_s_80	9733513	( B) Deletion analysis of the binding of JIP-1 to JNK1, MKK7, MLK3, and DLK.	bind
704	2	1034	6	10	NULL	0	NULL	CFTR	NULL		bind	NULL	efficiently	deltaF508 		GST-syn1AdeltaC	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_18_10972_s_157	9724814	( B) deltaF508 CFTR binds efficiently to GST-syn1AdeltaC when this mutant is processed at reduced temperature (see text for details).	bind
48604	1	1034	7	NULL	NULL	0	NULL	CFTR	GP		bind		efficiently	deltaF508		GST-syn1AdeltaC	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_18_10972_s_157	9724814	( B) deltaF508 CFTR binds efficiently to GST-syn1AdeltaC when this mutant is processed at reduced temperature (see text for details).	bind
705	1	1035	6	10	NULL	0	NULL	PICK1	NULL		bind	NULL		deltaNT 		GluR2	NULL		C-terminus		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_18_3266_s_81	16138078	( B) deltaNT PICK1 binds GluR2 C-terminus at maximal level in all [Ca2+]free tested.	bind
48606	1	1035	7	NULL	NULL	0	NULL	PICK1	GP		bind			deltaNT		 GluR2 	GP		C-terminus 		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_18_3266_s_81	16138078	( B) deltaNT PICK1 binds GluR2 C-terminus at maximal level in all [Ca2+]free tested.	bind
706	1	1036	6	NULL	NULL	0	NULL	GAPDH	NULL		bind	NULL				Siah1	NULL				NULL	MPTP treated mouse striatum	NULL	NULL	NULL	NULL	gw70_pnas_103_10_3887_s_67	16505364	( b) Deprenyl (DEP) inhibits the binding of GAPDH and Siah1 in MPTP treated mouse striatum.	bind
707	2	1036	6	10	NULL	0	NULL	DEP	NULL		inhibits	NULL				Statement 1	NULL				NULL	MPTP treated mouse striatum	NULL	NULL	NULL	NULL	gw70_pnas_103_10_3887_s_67	16505364	( b) Deprenyl (DEP) inhibits the binding of GAPDH and Siah1 in MPTP treated mouse striatum.	bind
51494	3	1036	6	10	NULL	0	NULL	DEP	NULL		is	NULL				Deprenyl 	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_103_10_3887_s_67	16505364	( b) Deprenyl (DEP) inhibits the binding of GAPDH and Siah1 in MPTP treated mouse striatum.	bind
48607	1	1036	7	3	NULL	0	NULL	GAPDH	GP		bind					Siah1	GP				NULL	MPTP treated mouse striatum	NULL	NULL	NULL	NULL	gw70_pnas_103_10_3887_s_67	16505364	( b) Deprenyl (DEP) inhibits the binding of GAPDH and Siah1 in MPTP treated mouse striatum.	bind
48608	2	1036	7	NULL	NULL	0	NULL	DEP	Chemical		inhibit					statement 1	GP				NULL	MPTP treated mouse striatum	NULL	NULL	NULL	NULL	gw70_pnas_103_10_3887_s_67	16505364	( b) Deprenyl (DEP) inhibits the binding of GAPDH and Siah1 in MPTP treated mouse striatum.	bind
48609	3	1036	7	NULL	NULL	0	NULL	DEP	Chemical		is					Deprenyl	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_10_3887_s_67	16505364	( b) Deprenyl (DEP) inhibits the binding of GAPDH and Siah1 in MPTP treated mouse striatum.	bind
708	1	1037	6	NULL	NULL	0	NULL	GAPDH	NULL		bind	NULL				Siah1	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_103_10_3887_s_39	16505364	( b) Deprenyl inhibits the binding of GAPDH and Siah1.	bind
709	2	1037	6	NULL	NULL	0	NULL	Deprenyl	NULL		inhibits	NULL				Statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_103_10_3887_s_39	16505364	( b) Deprenyl inhibits the binding of GAPDH and Siah1.	bind
48610	1	1037	7	NULL	NULL	0	NULL	GAPDH	GP		bind					Siah1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_10_3887_s_39	16505364	( b) Deprenyl inhibits the binding of GAPDH and Siah1.	bind
48611	2	1037	7	NULL	NULL	0	NULL	Deprenyl	Chemical		inhibit					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_10_3887_s_39	16505364	( b) Deprenyl inhibits the binding of GAPDH and Siah1.	bind
710	1	1039	6	NULL	NULL	0	NULL	BRCA1	NULL	purified	bind	NULL				STAT1alpha	NULL		C-terminus		NULL		0	NULL	NULL	NULL	gw60_pnas_97_10_5208_s_167	10792030	( B) Detection of binding of purified BRCA1 to STAT1alpha C terminus.	bind
48612	1	1039	7	NULL	NULL	0	NULL	BRCA1	GP	purified	bind					STAT1alpha	GP		C terminus		NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_10_5208_s_167	10792030	( B) Detection of binding of purified BRCA1 to STAT1alpha C terminus.	bind
711	1	1042	6	NULL	NULL	0	NULL	NHERF 	NULL		bind	NULL				beta2 receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_15_8496_s_110	9671706	( B) Determination of the binding affinity of NHERF for the beta2 receptor and P2Y1 receptor tails.	bind
712	2	1042	6	10	NULL	0	NULL	NHERF 	NULL		bind	NULL				P2Y1 receptor	NULL		 tails		NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_15_8496_s_110	9671706	( B) Determination of the binding affinity of NHERF for the beta2 receptor and P2Y1 receptor tails.	bind
48613	1	1042	7	NULL	NULL	0	NULL	NHERF	GP		bind					beta2 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_15_8496_s_110	9671706	( B) Determination of the binding affinity of NHERF for the beta2 receptor and P2Y1 receptor tails.	bind
48614	2	1042	7	NULL	NULL	0	NULL	NHERF	GP		bind					P2Y1 receptor	GP		tails		NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_15_8496_s_110	9671706	( B) Determination of the binding affinity of NHERF for the beta2 receptor and P2Y1 receptor tails.	bind
713	1	1043	6	NULL	NULL	0	NULL	UL28 protein	NULL		bind	NULL				pac1* DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_98_6_3086_s_155	11248036	( B) Determination of the binding affinity of UL28 protein for  pac1* DNA.	bind
48615	1	1043	7	NULL	NULL	0	NULL	UL28 protein	GP		bind					pac1* DNA	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_6_3086_s_155	11248036	( B) Determination of the binding affinity of UL28 protein for  pac1* DNA.	bind
714	1	1044	6	NULL	NULL	0	NULL	GGA3	NULL		bind	NULL		VHS (Vps27, Hrs, Stam) domain		cargo proteins	NULL				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_19_4423_s_26	16977309	( B) Diagram of GGA3 showing the VHS (Vps27, Hrs, Stam) domain, which binds to cargo  proteins, the GAT (GGA and TOM) domain, which binds to ARF1, the hinge segment, which  contains the autoregulatory acidic-dileucine motif and Ser388, and the GAE (gamma-adaptin ear) domain (Bonifacino, 2004) and GGA3 cargo.	bind
716	2	1044	6	NULL	NULL	0	NULL	GGA3	NULL		 bind	NULL		GAT (GGA and TOM) domain		ARF1	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_25_19_4423_s_26	16977309	( B) Diagram of GGA3 showing the VHS (Vps27, Hrs, Stam) domain, which binds to cargo  proteins, the GAT (GGA and TOM) domain, which binds to ARF1, the hinge segment, which  contains the autoregulatory acidic-dileucine motif and Ser388, and the GAE (gamma-adaptin ear) domain (Bonifacino, 2004) and GGA3 cargo.	bind
48618	1	1044	7	NULL	NULL	0	NULL	 GGA3	GP		bind			VHS domain		cargo proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_19_4423_s_26	16977309	( B) Diagram of GGA3 showing the VHS (Vps27, Hrs, Stam) domain, which binds to cargo  proteins, the GAT (GGA and TOM) domain, which binds to ARF1, the hinge segment, which  contains the autoregulatory acidic-dileucine motif and Ser388, and the GAE (gamma-adaptin ear) domain (Bonifacino, 2004) and GGA3 cargo.	bind
48619	2	1044	7	NULL	NULL	0	NULL	GGA3	GP		bind			GAT domain		ARF1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_19_4423_s_26	16977309	( B) Diagram of GGA3 showing the VHS (Vps27, Hrs, Stam) domain, which binds to cargo  proteins, the GAT (GGA and TOM) domain, which binds to ARF1, the hinge segment, which  contains the autoregulatory acidic-dileucine motif and Ser388, and the GAE (gamma-adaptin ear) domain (Bonifacino, 2004) and GGA3 cargo.	bind
48620	3	1044	7	NULL	NULL	0	NULL	GGA3	GP		contains			hinge segment				autoregulatory	acidic-dileucine motif 		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_19_4423_s_26	16977309	( B) Diagram of GGA3 showing the VHS (Vps27, Hrs, Stam) domain, which binds to cargo  proteins, the GAT (GGA and TOM) domain, which binds to ARF1, the hinge segment, which  contains the autoregulatory acidic-dileucine motif and Ser388, and the GAE (gamma-adaptin ear) domain (Bonifacino, 2004) and GGA3 cargo.	bind
48621	4	1044	7	NULL	NULL	0	NULL	GGA3	GP		bind			hinge segment					Ser388		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_19_4423_s_26	16977309	( B) Diagram of GGA3 showing the VHS (Vps27, Hrs, Stam) domain, which binds to cargo  proteins, the GAT (GGA and TOM) domain, which binds to ARF1, the hinge segment, which  contains the autoregulatory acidic-dileucine motif and Ser388, and the GAE (gamma-adaptin ear) domain (Bonifacino, 2004) and GGA3 cargo.	bind
48622	5	1044	7	NULL	NULL	0	NULL	GGA3	GP		contains			hinge segment						GAE domain	NULL		NULL	NULL	NULL	NULL	gw70_embo_25_19_4423_s_26	16977309	( B) Diagram of GGA3 showing the VHS (Vps27, Hrs, Stam) domain, which binds to cargo  proteins, the GAT (GGA and TOM) domain, which binds to ARF1, the hinge segment, which  contains the autoregulatory acidic-dileucine motif and Ser388, and the GAE (gamma-adaptin ear) domain (Bonifacino, 2004) and GGA3 cargo.	bind
48623	6	1044	7	NULL	NULL	0	NULL	GGA3	GP		bind			hinge segment		GGA3 cargo	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_19_4423_s_26	16977309	( B) Diagram of GGA3 showing the VHS (Vps27, Hrs, Stam) domain, which binds to cargo  proteins, the GAT (GGA and TOM) domain, which binds to ARF1, the hinge segment, which  contains the autoregulatory acidic-dileucine motif and Ser388, and the GAE (gamma-adaptin ear) domain (Bonifacino, 2004) and GGA3 cargo.	bind
48624	7	1044	7	NULL	NULL	0	NULL	GAE domain	GP		is					gamma-adaptin ear domain	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_19_4423_s_26	16977309	( B) Diagram of GGA3 showing the VHS (Vps27, Hrs, Stam) domain, which binds to cargo  proteins, the GAT (GGA and TOM) domain, which binds to ARF1, the hinge segment, which  contains the autoregulatory acidic-dileucine motif and Ser388, and the GAE (gamma-adaptin ear) domain (Bonifacino, 2004) and GGA3 cargo.	bind
718	1	1045	6	NULL	NULL	0	NULL	FtsZ peptide	NULL		bind	NULL				ZipA/M185	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_19_13_3179_s_297	10880432	( B) Difference electron density in the region of the FtsZ peptide bound to ZipA/M185.	bind
48616	1	1045	7	NULL	NULL	0	NULL	FtsZ peptide	GP		bind					 ZipA/M185	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_13_3179_s_297	10880432	( B) Difference electron density in the region of the FtsZ peptide bound to ZipA/M185.	bind
48617	1	1046	7	NULL	NULL	0	NULL	H3	GP	Dimethylation of	diminishes			 lysine 9		TRX 	GP	binding of	SET		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_17_2197_s_106	11544176	( B) Dimethylation of histone H3 on lysine 9 diminishes TRX SET binding.	bind
51495	2	1046	7	NULL	NULL	0	NULL	H3	GP		is a type of					histone	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_17_2197_s_106	11544176	( B) Dimethylation of histone H3 on lysine 9 diminishes TRX SET binding.	bind
812	1	1047	6	NULL	NULL	0	NULL	DinI	NULL		bind	NULL				RecA	NULL	activated			NULL		0	NULL	NULL	NULL	gw60_embo_20_5_1192_s_77	11230142	( B) DinI binds to activated RecA.	bind
48625	1	1047	7	NULL	NULL	0	NULL	DinI	GP		bind					RecA	GP	activated			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_5_1192_s_77	11230142	( B) DinI binds to activated RecA.	bind
875	2	1048	6	10	NULL	0	NULL	p50	NULL		bind	NULL					NULL			p50-specific DNA half site	NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_16_9268_s_158	12886018	( b) Direct  base-specific hydrogen-bonding contacts between p50 and p50-specific [[ DNA  half  site ]] observed in the x-ray structure of p50 homodimer bound to MHC-kappaB  DNA. ( c) Stacking interactions between residues in the linker (P243  and K241) and RNA bases  (G8 and G22) shown by van der  Waals surface model.	bind
877	1	1048	6	10	NULL	0	NULL	p50 homodimer	NULL		bind	NULL				MHC-kappaB DNA	NULL				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_16_9268_s_158	12886018	( b) Direct  base-specific hydrogen-bonding contacts between p50 and p50-specific [[ DNA  half  site ]] observed in the x-ray structure of p50 homodimer bound to MHC-kappaB  DNA. ( c) Stacking interactions between residues in the linker (P243  and K241) and RNA bases  (G8 and G22) shown by van der  Waals surface model.	bind
879	3	1048	6	10	NULL	0	NULL		NULL		interact	NULL		l	inker residues (P243 and K241)		NULL			\tRNA bases (G8 and G22)	NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_16_9268_s_158	12886018	( b) Direct  base-specific hydrogen-bonding contacts between p50 and p50-specific [[ DNA  half  site ]] observed in the x-ray structure of p50 homodimer bound to MHC-kappaB  DNA. ( c) Stacking interactions between residues in the linker (P243  and K241) and RNA bases  (G8 and G22) shown by van der  Waals surface model.	bind
48626	1	1048	7	NULL	NULL	0	NULL	p50 homodimer	GP		bind					MHC-kappaB DNA	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_16_9268_s_158	12886018	( b) Direct  base-specific hydrogen-bonding contacts between p50 and p50-specific [[ DNA  half  site ]] observed in the x-ray structure of p50 homodimer bound to MHC-kappaB  DNA. ( c) Stacking interactions between residues in the linker (P243  and K241) and RNA bases  (G8 and G22) shown by van der  Waals surface model.	bind
48627	2	1048	7	NULL	NULL	0	NULL	p50	GP		bind									p50-specific DNA half site	NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_16_9268_s_158	12886018	( b) Direct  base-specific hydrogen-bonding contacts between p50 and p50-specific [[ DNA  half  site ]] observed in the x-ray structure of p50 homodimer bound to MHC-kappaB  DNA. ( c) Stacking interactions between residues in the linker (P243  and K241) and RNA bases  (G8 and G22) shown by van der  Waals surface model.	bind
48628	3	1048	7	10	NULL	0	NULL		NULL		interacts with	NULL			\tlinker residues (P243 and K241)		NULL			\tRNA bases (G8 and G22)	NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_16_9268_s_158	12886018	( b) Direct  base-specific hydrogen-bonding contacts between p50 and p50-specific [[ DNA  half  site ]] observed in the x-ray structure of p50 homodimer bound to MHC-kappaB  DNA. ( c) Stacking interactions between residues in the linker (P243  and K241) and RNA bases  (G8 and G22) shown by van der  Waals surface model.	bind
813	1	1049	6	NULL	NULL	0	NULL	Arp2/3	NULL		bind	NULL				GST-control	NULL		region fragments		NULL		0	NULL	NULL	NULL	gw60_science_290_5492_801_s_76	11052943	( B) Direct binding of Arp2/3 to GST fusions of  control region fragments ( 27).	bind
48629	1	1049	7	NULL	NULL	0	NULL	Arp2/3	GP		bind		directly						control region fragments		NULL		NULL	NULL	NULL	NULL	gw60_science_290_5492_801_s_76	11052943	( B) Direct binding of Arp2/3 to GST fusions of  control region fragments ( 27).	bind
814	1	1050	6	10	NULL	0	NULL	Pbs2	NULL		bind	NULL	directly	RSD-1		Ssk2	NULL		kinase domain		NULL		NULL	NULL	NULL	NULL	gw60_embo_22_14_3624_s_142	12853477	( B) Direct binding of Pbs2 RSD-I to the Ssk2 kinase domain.	bind
48630	1	1050	7	NULL	NULL	0	NULL	Pbs2 	GP		bind		directly	RSD-I		 Ssk2	GP		kinase domain		NULL		NULL	NULL	NULL	NULL	gw60_embo_22_14_3624_s_142	12853477	( B) Direct binding of Pbs2 RSD-I to the Ssk2 kinase domain.	bind
815	1	1051	6	10	NULL	0	NULL	GST-Lyn 	NULL	purified	bind	NULL	directly	SH3		integrin beta proteins	NULL		cytoplasmic tail		NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_23_13298_s_182	14593208	( B) Direct binding of purified GST-Lyn SH3 to integrin beta cytoplasmic tail proteins, assessed by ELISA: beta1A ( ), beta2( ), beta3( ), rbeta1A ( ), and rbeta3( ).	bind
48631	1	1051	7	NULL	NULL	0	NULL	GST-Lyn 	GP	purified	bind		directly	SH3		integrin beta proteins	GP		 cytoplasmic tail		NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_23_13298_s_182	14593208	( B) Direct binding of purified GST-Lyn SH3 to integrin beta cytoplasmic tail proteins, assessed by ELISA: beta1A ( ), beta2( ), beta3( ), rbeta1A ( ), and rbeta3( ).	bind
816	1	1052	6	NULL	NULL	0	NULL	DM	NULL		bind	NULL				DR	NULL				NULL	cell surface	0	NULL	NULL	NULL	gw60_embo_19_6_1241_s_61	10716924	( B) DM is bound to DR on the cell surface.	bind
48632	1	1052	7	NULL	NULL	0	NULL	DM	GP		bind					DR	GP				NULL	cell surface	NULL	NULL	NULL	NULL	gw60_embo_19_6_1241_s_61	10716924	( B) DM is bound to DR on the cell surface.	bind
817	1	1053	6	10	NULL	0	NULL	DN-14-3-3	NULL		bind	NULL				14-3-3zeta	NULL	native;;WT			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_3_349_s_48	10654934	( B) DN-14-3-3  binds to native WT-14-3-3zeta.	bind
48633	1	1053	7	NULL	NULL	0	NULL	DN-14-3-3	GP		bind					14-3-3zeta	GP	native;;WT			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_3_349_s_48	10654934	( B) DN-14-3-3  binds to native WT-14-3-3zeta.	bind
818	1	1054	6	NULL	NULL	0	NULL	RNAP components	NULL		bind	NULL				psbA2 DNA	NULL			upstream region	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_21_4658_s_153	12409456	( B) DNA binding of RNAP components to the  psbA2 upstream region.	bind
48634	1	1054	7	NULL	NULL	0	NULL	RNAP components	GP		bind					psbA2 DNA	GP			upstream region	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_21_4658_s_153	12409456	( B) DNA binding of RNAP components to the  psbA2 upstream region.	bind
819	1	1058	6	NULL	NULL	0	NULL	OhrR	NULL		bind	NULL				ohrA	NULL			Promoter	NULL		0	NULL	NULL	NULL	gw60_pnas_99_10_6690_s_115	11983871	( B) DNase I footprinting analysis of OhrR binding to the  ohrA (lanes 1-9) and  ohrA* (lanes 10-18) promoters.	bind
48635	1	1058	7	NULL	NULL	0	NULL	OhrR	GP		bind					ohrA	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_10_6690_s_115	11983871	( B) DNase I footprinting analysis of OhrR binding to the  ohrA (lanes 1-9) and  ohrA* (lanes 10-18) promoters.	bind
821	1	1059	6	NULL	NULL	0	NULL	TFIID	NULL		bind	NULL				joc	NULL			Promoter	NULL		0	NULL	NULL	NULL	gw60_genesdev_11_22_3020_s_53	9367984	( B) DNase I footprinting analysis of the binding of TFIID to the  joc promoter.	bind
48636	1	1059	7	NULL	NULL	0	NULL	TFIID 	GP		bind					joc	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_22_3020_s_53	9367984	( B) DNase I footprinting analysis of the binding of TFIID to the  joc promoter.	bind
822	1	1060	6	NULL	NULL	0	NULL	Dnmt3a	NULL		bind	NULL		PDH-like motif		H3 methylase	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_9_2305_s_85	12711675	( B) Dnmt3a binds H3 methylase activity through its conserved PDH-like motif.	bind
48637	1	1060	7	NULL	NULL	0	NULL	Dnmt3a	GP		bind			conserved PDH-like motif		H3 methylase	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_9_2305_s_85	12711675	( B) Dnmt3a binds H3 methylase activity through its conserved PDH-like motif.	bind
823	1	1061	6	10	NULL	0	NULL	Dnmt3L	NULL		bind	NULL				HDAC1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_17_3831_s_39	12202768	( B) Dnmt3L binds the histone deacetylase HDAC1 in GST pull-down experiments.	bind
51498	2	1061	6	10	NULL	0	NULL	HDAC1	NULL		is a type of	NULL				histone deacetylase	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_17_3831_s_39	12202768	( B) Dnmt3L binds the histone deacetylase HDAC1 in GST pull-down experiments.	bind
48638	1	1061	7	NULL	NULL	0	NULL	Dnmt3L	GP		bind					HDAC1 	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_17_3831_s_39	12202768	( B) Dnmt3L binds the histone deacetylase HDAC1 in GST pull-down experiments.	bind
48639	2	1061	7	NULL	NULL	0	NULL	HDAC1	GP		is a type of					histone deacetylase	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_17_3831_s_39	12202768	( B) Dnmt3L binds the histone deacetylase HDAC1 in GST pull-down experiments.	bind
824	1	1062	6	NULL	NULL	0	NULL	CDCA	NULL		bind	NULL				FXR	NULL				NULL		0	NULL	NULL	NULL	gw60_science_284_5418_1365_s_66	10334993	( B) Dose response analysis of CDCA binding to FXR.	bind
48640	1	1062	7	NULL	NULL	0	NULL	CDCA	GP		bind					FXR	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5418_1365_s_66	10334993	( B) Dose response analysis of CDCA binding to FXR.	bind
825	1	1063	6	10	NULL	0	NULL	CD1d	NULL		bind	NULL	dose dependently			PI	NULL				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_29_10685_s_88	15243159	( b) Dose-dependency of CD1d binding to PI.	bind
48641	1	1063	7	NULL	NULL	0	NULL	CD1d	GP		bind		dose-dependently			PI	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_29_10685_s_88	15243159	( b) Dose-dependency of CD1d binding to PI.	bind
826	1	1064	6	10	NULL	0	NULL	mAb 146B7	NULL	biotinylated	bind	NULL	dose dependently			statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_112_10_1571_s_135	14617758	( b) Dose-dependent binding of biotinylated mAb 146B7 (filled squares) to IL-15 bound  to Raji lymphoma cells expressing IL-15Ralpha was shown by flow cytometry.	bind
827	2	1064	6	NULL	NULL	0	NULL	Raji lymphoma cells	NULL		express	NULL				IL-15Ralpha	NULL				NULL		0	NULL	NULL	NULL	gw70_jclininvest_112_10_1571_s_135	14617758	( b) Dose-dependent binding of biotinylated mAb 146B7 (filled squares) to IL-15 bound  to Raji lymphoma cells expressing IL-15Ralpha was shown by flow cytometry.	bind
51499	3	1064	6	10	NULL	0	NULL	IL-15	NULL		bind	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jclininvest_112_10_1571_s_135	14617758	( b) Dose-dependent binding of biotinylated mAb 146B7 (filled squares) to IL-15 bound  to Raji lymphoma cells expressing IL-15Ralpha was shown by flow cytometry.	bind
48642	3	1064	7	NULL	NULL	0	NULL	mAb 146B7	GP	biotinylated 	bind		dose-dependently			statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_112_10_1571_s_135	14617758	( b) Dose-dependent binding of biotinylated mAb 146B7 (filled squares) to IL-15 bound  to Raji lymphoma cells expressing IL-15Ralpha was shown by flow cytometry.	bind
48643	1	1064	7	NULL	NULL	0	NULL	Raji lymphoma cells	Cell		express					IL-15Ralpha	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_112_10_1571_s_135	14617758	( b) Dose-dependent binding of biotinylated mAb 146B7 (filled squares) to IL-15 bound  to Raji lymphoma cells expressing IL-15Ralpha was shown by flow cytometry.	bind
48644	2	1064	7	NULL	NULL	0	NULL	IL-15	GP		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_112_10_1571_s_135	14617758	( b) Dose-dependent binding of biotinylated mAb 146B7 (filled squares) to IL-15 bound  to Raji lymphoma cells expressing IL-15Ralpha was shown by flow cytometry.	bind
828	1	1065	6	10	NULL	0	NULL	CFTR	NULL	recombinant;;wild-type	bind	NULL	dose dependently			GST-syn1AH3	NULL	isolated	H3 domain		NULL	COS 7 cell lysates	NULL	NULL	NULL	NULL	gw60_pnas_95_18_10972_s_131	9724814	( B) Dose-dependent binding of CFTR to isolated H3 domain (GST-syn1AH3) in pull-down assay performed on COS 7 cell lysates expressing recombinant wild-type CFTR.	bind
48645	1	1065	7	NULL	NULL	0	NULL	CFTR	GP	recombinant;;wild-type	bind		dose dependently			GST-syn1AH3	GP	isolated	H3 domain		NULL	COS 7 cell lysates	NULL	NULL	NULL	NULL	gw60_pnas_95_18_10972_s_131	9724814	( B) Dose-dependent binding of CFTR to isolated H3 domain (GST-syn1AH3) in pull-down assay performed on COS 7 cell lysates expressing recombinant wild-type CFTR.	bind
829	1	1066	6	NULL	NULL	0	NULL	IP3	NULL		bind	NULL					NULL		PH domain		NULL		0	NULL	NULL	NULL	gw60_science_284_5419_1527_s_34	10348740	( B) Dose-dependent inhibition ( ) of PIP2 binding of the PH domain (2 muM) and estimated IP3 binding to the PH domain ( ) ( n = 3).	bind
830	2	1066	6	NULL	NULL	0	NULL	PIP2	NULL		bind	NULL					NULL		PH domain		NULL		0	NULL	NULL	NULL	gw60_science_284_5419_1527_s_34	10348740	( B) Dose-dependent inhibition ( ) of PIP2 binding of the PH domain (2 muM) and estimated IP3 binding to the PH domain ( ) ( n = 3).	bind
48646	1	1066	7	NULL	NULL	0	NULL	PIP2	GP		bind								PH domain		NULL		NULL	NULL	NULL	NULL	gw60_science_284_5419_1527_s_34	10348740	( B) Dose-dependent inhibition ( ) of PIP2 binding of the PH domain (2 muM) and estimated IP3 binding to the PH domain ( ) ( n = 3).	bind
48647	2	1066	7	NULL	NULL	0	NULL	IP3	Chemical		bind								PH domain		NULL		NULL	NULL	NULL	NULL	gw60_science_284_5419_1527_s_34	10348740	( B) Dose-dependent inhibition ( ) of PIP2 binding of the PH domain (2 muM) and estimated IP3 binding to the PH domain ( ) ( n = 3).	bind
832	1	1067	6	NULL	NULL	0	NULL	Pfu polymerase	NULL		bind	NULL				ssU	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_96_16_9045_s_127	10430892	( b) Dose-response curve for binding of  Pfu polymerase to ssU.	bind
48648	1	1067	7	NULL	NULL	0	NULL	Pfu polymerase	GP		bind					ssU	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_16_9045_s_127	10430892	( b) Dose-response curve for binding of  Pfu polymerase to ssU.	bind
837	1	1068	6	NULL	NULL	0	NULL	OspA-N40	NULL	FITC-labeled	bind	NULL				TGE	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_106_4_561_s_62	10953031	( b) Dose-response curves are presented for FITC-labeled OspA-N40, OspC, and BSA binding to TGE.	bind
838	2	1068	6	NULL	NULL	0	NULL	OspC	NULL	FITC-labeled	bind	NULL				TGE	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_106_4_561_s_62	10953031	( b) Dose-response curves are presented for FITC-labeled OspA-N40, OspC, and BSA binding to TGE.	bind
839	3	1068	6	NULL	NULL	0	NULL	BSA	NULL	FITC-labeled	bind	NULL				TGE	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_106_4_561_s_62	10953031	( b) Dose-response curves are presented for FITC-labeled OspA-N40, OspC, and BSA binding to TGE.	bind
48649	1	1068	7	NULL	NULL	0	NULL	OspA-N40	GP	FITC-labeled 	bind									TGE	NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_106_4_561_s_62	10953031	( b) Dose-response curves are presented for FITC-labeled OspA-N40, OspC, and BSA binding to TGE.	bind
48650	2	1068	7	NULL	NULL	0	NULL	OspC	GP	FITC-labeled 	bind									TGE	NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_106_4_561_s_62	10953031	( b) Dose-response curves are presented for FITC-labeled OspA-N40, OspC, and BSA binding to TGE.	bind
48651	3	1068	7	NULL	NULL	0	NULL	BSA	GP	FITC-labeled	bind									TGE	NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_106_4_561_s_62	10953031	( b) Dose-response curves are presented for FITC-labeled OspA-N40, OspC, and BSA binding to TGE.	bind
843	3	1069	6	10	NULL	0	NULL	Fibrinogen	NULL		bind	NULL				alphaIIb	NULL	mutant	G972N		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1424_s_135	15671157	( B) Dot plots of fibrinogen and anti-beta3 mouse mAb SSA6 binding to cells expressing the disruptive alphaIIb TM domain mutants G972N, G976L, and G976A and the permissive mutation L983A.	bind
844	7	1069	6	10	NULL	0	NULL	SSA6	NULL		bind	NULL				alphaIIb	NULL	mutant	G976A		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1424_s_135	15671157	( B) Dot plots of fibrinogen and anti-beta3 mouse mAb SSA6 binding to cells expressing the disruptive alphaIIb TM domain mutants G972N, G976L, and G976A and the permissive mutation L983A.	bind
1255	4	1069	6	10	NULL	0	NULL	Fibrinogen	NULL		bind	NULL				alphaIIb	NULL	mutant	G976L		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1424_s_135	15671157	( B) Dot plots of fibrinogen and anti-beta3 mouse mAb SSA6 binding to cells expressing the disruptive alphaIIb TM domain mutants G972N, G976L, and G976A and the permissive mutation L983A.	bind
1256	5	1069	6	10	NULL	0	NULL	Fibrinogen	NULL		bind	NULL				alphaIIb	NULL	mutant	G976A		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1424_s_135	15671157	( B) Dot plots of fibrinogen and anti-beta3 mouse mAb SSA6 binding to cells expressing the disruptive alphaIIb TM domain mutants G972N, G976L, and G976A and the permissive mutation L983A.	bind
1257	6	1069	6	10	NULL	0	NULL	Fibrinogen	NULL		bind	NULL				alphaIIb	NULL	mutant	L983A		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1424_s_135	15671157	( B) Dot plots of fibrinogen and anti-beta3 mouse mAb SSA6 binding to cells expressing the disruptive alphaIIb TM domain mutants G972N, G976L, and G976A and the permissive mutation L983A.	bind
1258	8	1069	6	NULL	NULL	0	NULL	SSA6	NULL	mouse mAb	bind	NULL				alphaIIb	NULL		TM domain mutant L983A		NULL		0	NULL	NULL	NULL	gw70_pnas_102_5_1424_s_135	15671157	( B) Dot plots of fibrinogen and anti-beta3 mouse mAb SSA6 binding to cells expressing the disruptive alphaIIb TM domain mutants G972N, G976L, and G976A and the permissive mutation L983A.	bind
1259	9	1069	6	NULL	NULL	0	NULL	SSA6	NULL	mouse mAb	bind	NULL				alphaIIb	NULL		TM domain mutant G976L		NULL		0	NULL	NULL	NULL	gw70_pnas_102_5_1424_s_135	15671157	( B) Dot plots of fibrinogen and anti-beta3 mouse mAb SSA6 binding to cells expressing the disruptive alphaIIb TM domain mutants G972N, G976L, and G976A and the permissive mutation L983A.	bind
1260	10	1069	6	NULL	NULL	0	NULL	SSA6	NULL	mouse mAb	bind	NULL				alphaIIb	NULL		TM domain mutant G972N		NULL		0	NULL	NULL	NULL	gw70_pnas_102_5_1424_s_135	15671157	( B) Dot plots of fibrinogen and anti-beta3 mouse mAb SSA6 binding to cells expressing the disruptive alphaIIb TM domain mutants G972N, G976L, and G976A and the permissive mutation L983A.	bind
48656	1	1069	7	NULL	NULL	0	NULL	fibrinogen	GP		bind					alphaIIb 	GP	mutant	G972N		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1424_s_135	15671157	( B) Dot plots of fibrinogen and anti-beta3 mouse mAb SSA6 binding to cells expressing the disruptive alphaIIb TM domain mutants G972N, G976L, and G976A and the permissive mutation L983A.	bind
48657	2	1069	7	NULL	NULL	0	NULL	fibrinogen	GP		bind					alphaIIb	GP	mutant	G976L		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1424_s_135	15671157	( B) Dot plots of fibrinogen and anti-beta3 mouse mAb SSA6 binding to cells expressing the disruptive alphaIIb TM domain mutants G972N, G976L, and G976A and the permissive mutation L983A.	bind
48658	3	1069	7	NULL	NULL	0	NULL	fibrinogen	GP		bind					alphaIIb	GP	mutant	G976A		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1424_s_135	15671157	( B) Dot plots of fibrinogen and anti-beta3 mouse mAb SSA6 binding to cells expressing the disruptive alphaIIb TM domain mutants G972N, G976L, and G976A and the permissive mutation L983A.	bind
48659	4	1069	7	NULL	NULL	0	NULL	fibrinogen	GP		bind					alphaIIb	GP	mutant	L983A		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1424_s_135	15671157	( B) Dot plots of fibrinogen and anti-beta3 mouse mAb SSA6 binding to cells expressing the disruptive alphaIIb TM domain mutants G972N, G976L, and G976A and the permissive mutation L983A.	bind
48660	5	1069	7	NULL	NULL	0	NULL	anti-beta3 mouse mAb SSA6 	GP		bind					alphaIIb	GP	mutant	TM domain G972N		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1424_s_135	15671157	( B) Dot plots of fibrinogen and anti-beta3 mouse mAb SSA6 binding to cells expressing the disruptive alphaIIb TM domain mutants G972N, G976L, and G976A and the permissive mutation L983A.	bind
48661	6	1069	7	NULL	NULL	0	NULL	anti-beta3 mouse mAb SSA6	GP		bind					alphaIIb	GP	mutant	TM domain G976L		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1424_s_135	15671157	( B) Dot plots of fibrinogen and anti-beta3 mouse mAb SSA6 binding to cells expressing the disruptive alphaIIb TM domain mutants G972N, G976L, and G976A and the permissive mutation L983A.	bind
48662	7	1069	7	NULL	NULL	0	NULL	anti-beta3 mouse mAb SSA6	GP		bind					alphaIIb	GP	mutant	TM domain G976A		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1424_s_135	15671157	( B) Dot plots of fibrinogen and anti-beta3 mouse mAb SSA6 binding to cells expressing the disruptive alphaIIb TM domain mutants G972N, G976L, and G976A and the permissive mutation L983A.	bind
48663	8	1069	7	NULL	NULL	0	NULL	anti-beta3 mouse mAb SSA6	GP		bind					alphaIIb	GP	mutant	L983A		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1424_s_135	15671157	( B) Dot plots of fibrinogen and anti-beta3 mouse mAb SSA6 binding to cells expressing the disruptive alphaIIb TM domain mutants G972N, G976L, and G976A and the permissive mutation L983A.	bind
845	1	1070	6	NULL	NULL	0	NULL	Fibrinogen	NULL		bind	NULL				alphaIIbbeta3	NULL	human wild type			NULL		0	NULL	NULL	NULL	gw70_pnas_102_5_1424_s_101	15671157	( B) Dot plots of fibrinogen and anti-beta3 mouse mAb SSA6 binding to cells expressing WT human alphaIIbbeta3 and the alphaIIb mutant G972N.	bind
846	2	1070	6	NULL	NULL	0	NULL	SSA6	NULL	mouse mAb	bind	NULL				alphaIIbbeta3	NULL	human wild type			NULL		0	NULL	NULL	NULL	gw70_pnas_102_5_1424_s_101	15671157	( B) Dot plots of fibrinogen and anti-beta3 mouse mAb SSA6 binding to cells expressing WT human alphaIIbbeta3 and the alphaIIb mutant G972N.	bind
847	3	1070	6	NULL	NULL	0	NULL	Fibrinogen	NULL		bind	NULL				alphaIIb	NULL	human	TM domain mutant G972N		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1424_s_101	15671157	( B) Dot plots of fibrinogen and anti-beta3 mouse mAb SSA6 binding to cells expressing WT human alphaIIbbeta3 and the alphaIIb mutant G972N.	bind
848	4	1070	6	NULL	NULL	0	NULL	SSA6	NULL	mouse mAb	bind	NULL				alphaIIb	NULL	human	TM domain mutant G972N		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1424_s_101	15671157	( B) Dot plots of fibrinogen and anti-beta3 mouse mAb SSA6 binding to cells expressing WT human alphaIIbbeta3 and the alphaIIb mutant G972N.	bind
48664	1	1070	7	NULL	NULL	0	NULL	cells	Cell		express					alphaIIbbeta3	GP	WT;; human			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1424_s_101	15671157	( B) Dot plots of fibrinogen and anti-beta3 mouse mAb SSA6 binding to cells expressing WT human alphaIIbbeta3 and the alphaIIb mutant G972N.	bind
48665	2	1070	7	NULL	NULL	0	NULL	cells	Cell		express					alphaIIb	GP	mutant	G972N		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1424_s_101	15671157	( B) Dot plots of fibrinogen and anti-beta3 mouse mAb SSA6 binding to cells expressing WT human alphaIIbbeta3 and the alphaIIb mutant G972N.	bind
48666	3	1070	7	NULL	NULL	0	NULL	fibrinogen	GP		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1424_s_101	15671157	( B) Dot plots of fibrinogen and anti-beta3 mouse mAb SSA6 binding to cells expressing WT human alphaIIbbeta3 and the alphaIIb mutant G972N.	bind
48667	4	1070	7	NULL	NULL	0	NULL	fibrinogen	GP		bind					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1424_s_101	15671157	( B) Dot plots of fibrinogen and anti-beta3 mouse mAb SSA6 binding to cells expressing WT human alphaIIbbeta3 and the alphaIIb mutant G972N.	bind
48668	5	1070	7	NULL	NULL	0	NULL	anti-beta3 mouse mAb SSA6	GP		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1424_s_101	15671157	( B) Dot plots of fibrinogen and anti-beta3 mouse mAb SSA6 binding to cells expressing WT human alphaIIbbeta3 and the alphaIIb mutant G972N.	bind
48669	6	1070	7	NULL	NULL	0	NULL	anti-beta3 mouse mAb SSA6	GP		bind					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1424_s_101	15671157	( B) Dot plots of fibrinogen and anti-beta3 mouse mAb SSA6 binding to cells expressing WT human alphaIIbbeta3 and the alphaIIb mutant G972N.	bind
849	1	1071	6	NULL	NULL	0	NULL	HSF	NULL		bind	NULL				H3	NULL	acetylated		heat shock promoter elements	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_23_3003_s_168	11114889	( B) During heat shock, the heat shock transcription factor (HSF) binds to acetylated H3 and H4 residues at the heat shock promoter elements.	bind
851	2	1071	6	NULL	NULL	0	NULL	HSF	NULL		bind	NULL				H4	NULL	acetylated		heat shock promoter elements	NULL		0	NULL	NULL	NULL	gw60_genesdev_14_23_3003_s_168	11114889	( B) During heat shock, the heat shock transcription factor (HSF) binds to acetylated H3 and H4 residues at the heat shock promoter elements.	bind
852	3	1071	6	NULL	NULL	0	NULL	HSF	NULL		is	NULL				heat shock transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_14_23_3003_s_168	11114889	( B) During heat shock, the heat shock transcription factor (HSF) binds to acetylated H3 and H4 residues at the heat shock promoter elements.	bind
48670	1	1071	7	NULL	NULL	0	NULL	HSF	GP		bind					H3 residues	GP	 acetylated		 heat shock promoter element	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_23_3003_s_168	11114889	( B) During heat shock, the heat shock transcription factor (HSF) binds to acetylated H3 and H4 residues at the heat shock promoter elements.	bind
48671	2	1071	7	NULL	NULL	0	NULL	HSF	GP		bind					H4 residues	GP	acetylated		 heat shock promoter element	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_23_3003_s_168	11114889	( B) During heat shock, the heat shock transcription factor (HSF) binds to acetylated H3 and H4 residues at the heat shock promoter elements.	bind
48672	3	1071	7	NULL	NULL	0	NULL	HSF	GP		is					heat shock transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_23_3003_s_168	11114889	( B) During heat shock, the heat shock transcription factor (HSF) binds to acetylated H3 and H4 residues at the heat shock promoter elements.	bind
855	1	1072	6	NULL	NULL	0	NULL	PDGF	NULL		bind	NULL				PDGF-R	NULL				NULL		0	NULL	NULL	NULL	gw60_science_297_5583_948_s_26	12169717	( B) During switch activation, the binding of PDGF to its receptor (PDGF-R) leads to the activation of Ras.	bind
857	2	1072	6	10	NULL	0	NULL	Statement 1	NULL		leads to	NULL				Ras	NULL	activation of			NULL		NULL	NULL	NULL	NULL	gw60_science_297_5583_948_s_26	12169717	( B) During switch activation, the binding of PDGF to its receptor (PDGF-R) leads to the activation of Ras.	bind
858	3	1072	6	NULL	NULL	0	NULL	Statement 1	NULL		occurs during	NULL				switch activation	NULL				NULL		0	NULL	NULL	NULL	gw60_science_297_5583_948_s_26	12169717	( B) During switch activation, the binding of PDGF to its receptor (PDGF-R) leads to the activation of Ras.	bind
860	4	1072	6	NULL	NULL	0	NULL	statement 2	NULL		occurs during	NULL				switch activation	NULL				NULL		0	NULL	NULL	NULL	gw60_science_297_5583_948_s_26	12169717	( B) During switch activation, the binding of PDGF to its receptor (PDGF-R) leads to the activation of Ras.	bind
48673	1	1072	7	NULL	NULL	0	NULL	PDGF	GP		bind					PDGF-R	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_297_5583_948_s_26	12169717	( B) During switch activation, the binding of PDGF to its receptor (PDGF-R) leads to the activation of Ras.	bind
48674	2	1072	7	NULL	NULL	0	NULL	statement 1	Process		leads to					Ras	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_science_297_5583_948_s_26	12169717	( B) During switch activation, the binding of PDGF to its receptor (PDGF-R) leads to the activation of Ras.	bind
48675	3	1072	7	NULL	NULL	0	NULL	statement 1	Process		occurs during					switch activation	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_297_5583_948_s_26	12169717	( B) During switch activation, the binding of PDGF to its receptor (PDGF-R) leads to the activation of Ras.	bind
48676	4	1072	7	NULL	NULL	0	NULL	PDGF-R	GP		is					PDGF receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_297_5583_948_s_26	12169717	( B) During switch activation, the binding of PDGF to its receptor (PDGF-R) leads to the activation of Ras.	bind
972	1	1073	6	NULL	NULL	0	NULL	c-Jun	NULL		bind	NULL				TNF	NULL			TRE site	NULL	RAW 264.7 cells	0	NULL	NULL	NULL	gw60_jclininvest_104_4_503_s_214	10449442	( b) E2 treatment of RAW 264.7 cells decreases the binding of c-Jun and JunD to a probe containing an exact copy of the TRE site found in the TNF promoter.	bind
973	2	1073	6	NULL	NULL	0	NULL	JunD	NULL		bind	NULL				TNF	NULL			TRE site	NULL	RAW 264.7 cells	NULL	NULL	NULL	NULL	gw60_jclininvest_104_4_503_s_214	10449442	( b) E2 treatment of RAW 264.7 cells decreases the binding of c-Jun and JunD to a probe containing an exact copy of the TRE site found in the TNF promoter.	bind
1106	3	1073	6	NULL	NULL	0	NULL	E2 	NULL		decreases 	NULL				Statement 1	NULL				NULL	RAW 264.7 cells	NULL	NULL	NULL	NULL	gw60_jclininvest_104_4_503_s_214	10449442	( b) E2 treatment of RAW 264.7 cells decreases the binding of c-Jun and JunD to a probe containing an exact copy of the TRE site found in the TNF promoter.	bind
1107	4	1073	6	NULL	NULL	0	NULL	E2	NULL		decreases 	NULL				Statement 2	NULL				NULL	RAW 264.7 cells	NULL	NULL	NULL	NULL	gw60_jclininvest_104_4_503_s_214	10449442	( b) E2 treatment of RAW 264.7 cells decreases the binding of c-Jun and JunD to a probe containing an exact copy of the TRE site found in the TNF promoter.	bind
48677	1	1073	7	NULL	NULL	0	NULL	c-Jun	GP		bind					TNF	GP			TRE site in promoter	NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_104_4_503_s_214	10449442	( b) E2 treatment of RAW 264.7 cells decreases the binding of c-Jun and JunD to a probe containing an exact copy of the TRE site found in the TNF promoter.	bind
48678	2	1073	7	NULL	NULL	0	NULL	JunD	GP		bind					TNF	GP			TRE site in promoter	NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_104_4_503_s_214	10449442	( b) E2 treatment of RAW 264.7 cells decreases the binding of c-Jun and JunD to a probe containing an exact copy of the TRE site found in the TNF promoter.	bind
48679	3	1073	7	NULL	NULL	0	NULL	RAW 264.7 cells	Cell		treated with					E2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_104_4_503_s_214	10449442	( b) E2 treatment of RAW 264.7 cells decreases the binding of c-Jun and JunD to a probe containing an exact copy of the TRE site found in the TNF promoter.	bind
48680	4	1073	7	NULL	NULL	0	NULL	statement 3	Process		decrease					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_104_4_503_s_214	10449442	( b) E2 treatment of RAW 264.7 cells decreases the binding of c-Jun and JunD to a probe containing an exact copy of the TRE site found in the TNF promoter.	bind
48681	5	1073	7	NULL	NULL	0	NULL	statement 3	Process		decrease					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_104_4_503_s_214	10449442	( b) E2 treatment of RAW 264.7 cells decreases the binding of c-Jun and JunD to a probe containing an exact copy of the TRE site found in the TNF promoter.	bind
1003	1	1074	6	NULL	NULL	0	NULL	CRP	NULL		bind	NULL				PAPC	NULL	oxidized			NULL		0	NULL	NULL	NULL	gw60_pnas_99_20_13043_s_108	12244213	( B) Effect of calcium on the binding of CRP to oxidized PAPC.	bind
48682	1	1074	7	NULL	NULL	0	NULL	CRP	GP		bind					PAPC	Chemical	oxidized			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_20_13043_s_108	12244213	( B) Effect of calcium on the binding of CRP to oxidized PAPC.	bind
1004	1	1075	6	NULL	NULL	0	NULL	OspA	NULL	labeled	bind	NULL				TGE	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_106_4_561_s_71	10953031	( b) Effect of excess unlabeled OspA on the binding of labeled OspA to TGE.	bind
48683	1	1075	7	NULL	NULL	0	NULL	 OspA 	GP	labeled	bind					TGE					NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_106_4_561_s_71	10953031	( b) Effect of excess unlabeled OspA on the binding of labeled OspA to TGE.	bind
1011	1	1076	6	NULL	NULL	0	NULL	nuclear protein	NULL		bind	NULL				oligonucleotide	NULL			GC-box	NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_27_2_252_s_168	16150893	( B) Effect of mithramycin A on the binding of nuclear proteins to the GC-box oligonucleotide.	bind
48684	1	1076	7	NULL	NULL	0	NULL	nuclear proteins	GP		bind					oligonucleotide	NucleicAcid			GC-box	NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_2_252_s_168	16150893	( B) Effect of mithramycin A on the binding of nuclear proteins to the GC-box oligonucleotide.	bind
1012	1	1078	6	NULL	NULL	0	NULL	GDP	NULL		bind	NULL				Rac1	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_96_9_4826_s_116	10220378	( B) Effect of the DH domain mutant Ras-GRF1(DH(-)) on GDP binding to Rac1.	bind
48685	1	1078	7	NULL	NULL	0	NULL	GDP	Chemical		bind					Rac1	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_9_4826_s_116	10220378	( B) Effect of the DH domain mutant Ras-GRF1(DH(-)) on GDP binding to Rac1.	bind
1013	1	1079	6	NULL	NULL	0	NULL	OspA	NULL		bind	NULL				TGE	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_106_4_561_s_214	10953031	( b) Effect of trypsin treatment on OspA binding to TGE.	bind
48686	1	1079	7	NULL	NULL	0	NULL	OspA	GP		bind					TGE	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_106_4_561_s_214	10953031	( b) Effect of trypsin treatment on OspA binding to TGE.	bind
1867	2	1080	6	10	NULL	0	NULL	cabin1	NULL		associate with	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_12_2104_s_184	15902271	( B) Effects of calcium and CaMKIV on association of Cabin1 with MEF2 bound to the endogenous  IL-2 promoter.	bind
1868	1	1080	6	10	NULL	0	NULL	MEF2	NULL		bind	NULL				IL-2	NULL	endogenous		promoter	NULL		NULL	NULL	NULL	NULL	gw70_embo_24_12_2104_s_184	15902271	( B) Effects of calcium and CaMKIV on association of Cabin1 with MEF2 bound to the endogenous  IL-2 promoter.	bind
48687	1	1080	7	NULL	NULL	0	NULL	MEF2	GP		bind					IL-2	GP	endogenous		promoter	NULL		NULL	NULL	NULL	NULL	gw70_embo_24_12_2104_s_184	15902271	( B) Effects of calcium and CaMKIV on association of Cabin1 with MEF2 bound to the endogenous  IL-2 promoter.	bind
48688	2	1080	7	NULL	NULL	0	NULL	Cabin1	GP		associate with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_12_2104_s_184	15902271	( B) Effects of calcium and CaMKIV on association of Cabin1 with MEF2 bound to the endogenous  IL-2 promoter.	bind
1041	1	1081	6	NULL	NULL	0	NULL	PCNA	NULL		bind	NULL				GST-pol	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_23_19_3886_s_215	15359278	( B) Effects of different salt concentrations on the binding of PCNA to GST-pol  (left) and on PCNA elution from GST-pol  (right).	bind
48689	1	1081	7	NULL	NULL	0	NULL	 PCNA	GP		bind					GST-pol	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_19_3886_s_215	15359278	( B) Effects of different salt concentrations on the binding of PCNA to GST-pol  (left) and on PCNA elution from GST-pol  (right).	bind
58423	1	1082	7	NULL	NULL	0	NULL	forskolin	GP		induce					CREB	GP	activation dependent on			NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_7_3652_s_118	10097092	( B) Effects of p/CIP holoprotein and p/CIP ligand binding interaction domain on forskolin-induced CREB-dependent activation as described ( 3).	bind
1042	1	1083	6	NULL	NULL	0	NULL	Dsk2p	NULL		bind	NULL				polyubiquitin	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_2_745_s_137	11805328	( B) Effects of Ub lysine mutants on binding between Dsk2p and polyubiquitin.	bind
48691	1	1083	7	NULL	NULL	0	NULL	Dsk2p	GP		bind					polyubiquitin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_2_745_s_137	11805328	( B) Effects of Ub lysine mutants on binding between Dsk2p and polyubiquitin.	bind
1043	1	1084	6	NULL	NULL	0	NULL	TVA-EGF	NULL		bind	NULL				M5 cells	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_12_7063_s_90	9618539	( B) EGF competes for TVA-EGF binding to M5 cells.	bind
1044	2	1084	6	10	NULL	0	NULL	EGF	NULL		bind	NULL				M5 cells	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_12_7063_s_90	9618539	( B) EGF competes for TVA-EGF binding to M5 cells.	bind
51518	3	1084	6	10	NULL	0	NULL	statement 2	NULL		competes with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_12_7063_s_90	9618539	( B) EGF competes for TVA-EGF binding to M5 cells.	bind
48692	1	1084	7	NULL	NULL	0	NULL	TVA-EGF	GP		bind					M5 cells	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_12_7063_s_90	9618539	( B) EGF competes for TVA-EGF binding to M5 cells.	bind
48693	2	1084	7	NULL	NULL	0	NULL	EGF 	GP		bind					M5 cells	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_12_7063_s_90	9618539	( B) EGF competes for TVA-EGF binding to M5 cells.	bind
48694	3	1084	7	NULL	NULL	0	NULL	statement 2	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_12_7063_s_90	9618539	( B) EGF competes for TVA-EGF binding to M5 cells.	bind
1045	1	1088	6	10	NULL	0	NULL	Desrt	NULL	recombinant	bind	NULL		ARID domain		(TTA)9 oligonucleotide	NULL				NULL		NULL	NULL	NULL	NULL	gw60_genomeres_11_8_1327_s_38	11483573	( B) Electrophoretic mobility shift assay (EMSA) of recombinant Desrt-ARID domain binding to a (TTA)9 oligonucleotide (lane  3).	bind
48695	1	1088	7	NULL	NULL	0	NULL	Desrt	GP	recombinant	bind			ARID domain 		(TTA)9 oligonucleotide	GP				NULL		NULL	NULL	NULL	NULL	gw60_genomeres_11_8_1327_s_38	11483573	( B) Electrophoretic mobility shift assay (EMSA) of recombinant Desrt-ARID domain binding to a (TTA)9 oligonucleotide (lane  3).	bind
1046	1	1090	6	10	NULL	0	NULL	CBFA1	NULL		bind	NULL				OSE2 oligonucleotide	NULL				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_9_2254_s_260	11331591	( B) Electrophoretic mobility shift assays show CBFA1 binding to an OSE2 oligonucleotide, both in the absence or presence of Smad3 and Smad4.	bind
48696	1	1090	7	NULL	NULL	0	NULL	CBFA1	GP		bind					OSE2 oligonucleotide	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_9_2254_s_260	11331591	( B) Electrophoretic mobility shift assays show CBFA1 binding to an OSE2 oligonucleotide, both in the absence or presence of Smad3 and Smad4.	bind
1077	1	1091	6	10	NULL	0	NULL	MEF2C	NULL		bind	NULL				PGC-1 alpha	NULL	putative		MEF2 sites in proximal promotor of	NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_4_1711_s_155	12578979	( B) Electrophoretic mobility-shift assay for binding of MEF2C to the putative MEF2 sites  of the 3.1-kb proximal  PGC-1alpha promoter.	bind
48697	1	1091	7	NULL	NULL	0	NULL	MEF2C	GP		bind					PGC-1alpha	GP	putative		MEF2 sites in proximal promotor of	NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_4_1711_s_155	12578979	( B) Electrophoretic mobility-shift assay for binding of MEF2C to the putative MEF2 sites  of the 3.1-kb proximal  PGC-1alpha promoter.	bind
831	1	1092	5	10	NULL	0	NULL	MEF2C	GP		bind					PGC-1alpha	GP			putative MEF2 sites of proximal promoter	NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_4_1711_s_155	12578979	( B) Electrophoretic mobility-shift assay for binding of MEF2C to the putative MEF2 sites of the 3.1-kb proximal  PGC-1alpha promoter.	bind
217	1	1092	7	10	NULL	0	NULL	MEF2C	GP		bind					PGC-1alpha 	GP			putative MEF2 sites of proximal promoter	NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_4_1711_s_155	12578979	( B) Electrophoretic mobility-shift assay for binding of MEF2C to the putative MEF2 sites of the 3.1-kb proximal  PGC-1alpha promoter.	bind
833	1	1093	5	10	NULL	0	NULL	Ab	GP		bind					BDNF	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_25_14702_s_48	11724927	( B) ELISA demonstrating the reduced binding of the Ab to BDNF after modification with the caging group and its successful reactivation by UV light.	bind
48715	2	1093	5	10	NULL	0	NULL	statement 1	Process		occurs after					caging group	Process	modification with			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_25_14702_s_48	11724927	( B) ELISA demonstrating the reduced binding of the Ab to BDNF after modification with the caging group and its successful reactivation by UV light.	bind
48716	3	1093	5	10	NULL	0	NULL	UV light			reactivates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_25_14702_s_48	11724927	( B) ELISA demonstrating the reduced binding of the Ab to BDNF after modification with the caging group and its successful reactivation by UV light.	bind
230	1	1093	7	10	NULL	0	NULL	Ab 	GP		bind					BDNF	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_25_14702_s_48	11724927	( B) ELISA demonstrating the reduced binding of the Ab to BDNF after modification with the caging group and its successful reactivation by UV light.	bind
231	2	1093	7	10	NULL	0	NULL	statement 1	Process		occurs after					caging group 	Process	modification with			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_25_14702_s_48	11724927	( B) ELISA demonstrating the reduced binding of the Ab to BDNF after modification with the caging group and its successful reactivation by UV light.	bind
232	3	1093	7	10	NULL	0	NULL	UV light			reactivates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_25_14702_s_48	11724927	( B) ELISA demonstrating the reduced binding of the Ab to BDNF after modification with the caging group and its successful reactivation by UV light.	bind
834	1	1094	5	10	NULL	0	NULL	RBP	GP		bind					TTR	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_17_4633_s_278	10469643	( B) Elution profile observed for mRBP in wild-type serum: essentially all RBP is bound to TTR.	bind
311	1	1094	7	10	NULL	0	NULL	RBP	GP		bind					TTR	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_17_4633_s_278	10469643	( B) Elution profile observed for mRBP in wild-type serum: essentially all RBP is bound to TTR.	bind
835	1	1095	5	10	NULL	0	NULL	Cdc20	GP		bind					APC	Cell				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_genesdev_15_24_3278_s_101	11751633	( B) Emi1 does not prevent Cdc20 binding to the APC in vitro.	bind
836	2	1095	5	10	NULL	0	NULL	Emi1	GP		does not prevent					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_24_3278_s_101	11751633	( B) Emi1 does not prevent Cdc20 binding to the APC in vitro.	bind
312	1	1095	7	10	NULL	0	NULL	Cdc20	GP		bind					APC	Cell				NULL	 in vitro	NULL	NULL	NULL	NULL	gw60_genesdev_15_24_3278_s_101	11751633	( B) Emi1 does not prevent Cdc20 binding to the APC in vitro.	bind
313	2	1095	7	10	NULL	0	NULL	Emi1	GP		does not prevent 					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_24_3278_s_101	11751633	( B) Emi1 does not prevent Cdc20 binding to the APC in vitro.	bind
840	1	1096	5	10	NULL	0	NULL	CaMKII	GP		phosphorylate					Emi2	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_3_608_s_65	16407128	( B) Emi2 binds the PBD of Plk1 after phosphorylation by CaMKII.	bind
841	2	1096	5	10	NULL	0	NULL	Emi2	GP		bind					Plk1	GP		PBD		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_3_608_s_65	16407128	( B) Emi2 binds the PBD of Plk1 after phosphorylation by CaMKII.	bind
842	3	1096	5	10	NULL	0	NULL	statement 2	Process		occurs after					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_3_608_s_65	16407128	( B) Emi2 binds the PBD of Plk1 after phosphorylation by CaMKII.	bind
314	1	1096	7	10	NULL	0	NULL	Emi2	GP		bind					Plk1	GP		PBD		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_3_608_s_65	16407128	( B) Emi2 binds the PBD of Plk1 after phosphorylation by CaMKII.	bind
315	2	1096	7	10	NULL	0	NULL	CaMKII	GP		phosphorylate					Emi2	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_3_608_s_65	16407128	( B) Emi2 binds the PBD of Plk1 after phosphorylation by CaMKII.	bind
48698	3	1096	7	10	NULL	0	NULL	statement 1	Process		occurs after					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_3_608_s_65	16407128	( B) Emi2 binds the PBD of Plk1 after phosphorylation by CaMKII.	bind
850	1	1097	5	10	NULL	0	NULL	nuclear protein	GP		bind					COX-2	GP			NF-IL-6 region of promoter	NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_4_1788_s_188	9465095	( B) EMSA of binding of nuclear protein to the NF-IL-6 region of the COX-2 promoter.	bind
317	1	1097	7	10	NULL	0	NULL	nuclear protein 	GP		binds to					COX-2	GP			NF-IL-6 promoter 	NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_4_1788_s_188	9465095	( B) EMSA of binding of nuclear protein to the NF-IL-6 region of the COX-2 promoter.	bind
853	1	1098	5	10	NULL	0	NULL	DLX1	GP		bind					Dlx5/ Dlx6	GP	specific		homeodomain binding motifs of intergenic enhancer	NULL	embryonic striatum in situ	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_32_3_884_s_178	14769946	( b) EMSA of embryonic striatum demonstrates DLX1 and DLX2 binding to specific homeodomain  binding motifs within the  Dlx5/ Dlx6 intergenic enhancer  in situ.	bind
854	2	1098	5	10	NULL	0	NULL	DLX2	GP		bind					Dlx5/ Dlx6	GP	specific		homeodomain binding motifs of intergenic enhancer	NULL	embryonic striatum in situ	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_32_3_884_s_178	14769946	( b) EMSA of embryonic striatum demonstrates DLX1 and DLX2 binding to specific homeodomain  binding motifs within the  Dlx5/ Dlx6 intergenic enhancer  in situ.	bind
335	1	1098	7	10	NULL	0	NULL	DLX1	GP		binds to 					Dlx5/Dlx6	GP	specific 		homeodomain binding motifs  within intergenic enhancer 	NULL	embryonic striatum in situ	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_32_3_884_s_178	14769946	( b) EMSA of embryonic striatum demonstrates DLX1 and DLX2 binding to specific homeodomain  binding motifs within the  Dlx5/ Dlx6 intergenic enhancer  in situ.	bind
338	2	1098	7	10	NULL	0	NULL	DLX2	GP		binds to					Dlx5/Dlx6 	GP	specific 		homeodomain binding motifs within intergenic enhancer	NULL	embryonic striatum in situ	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_32_3_884_s_178	14769946	( b) EMSA of embryonic striatum demonstrates DLX1 and DLX2 binding to specific homeodomain  binding motifs within the  Dlx5/ Dlx6 intergenic enhancer  in situ.	bind
856	1	1099	5	10	NULL	0	NULL	Akt	GP	endogenous	bind					acinus-S	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_20_3543_s_214	16177823	( B) Endogenous Akt binds to acinus-S.	bind
343	1	1099	7	10	NULL	0	NULL	Akt	GP	Endogenous	binds to					acinus-S	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_20_3543_s_214	16177823	( B) Endogenous Akt binds to acinus-S.	bind
859	1	1100	5	10	NULL	0	NULL	E2F	GP	endogenous	bind					BMI1	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_6_1745_s_149	16582100	( B) Endogenous E2F proteins bind to the  BMI1 promoter  in vivo.	bind
345	1	1100	7	10	NULL	0	NULL	E2F proteins 	GP	endogenous	binds to 					BMI1	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_6_1745_s_149	16582100	( B) Endogenous E2F proteins bind to the  BMI1 promoter  in vivo.	bind
861	1	1101	5	10	NULL	0	NULL	FoxO3a	GP	endogenous	bind					cyclin D2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_embo_23_14_2830_s_161	15241468	( B) Endogenous FoxO3a binds to the  cyclin D2 promoter upon inhibition of PI3-kinase.	bind
862	2	1101	5	10	NULL	0	NULL	statement 1	Process		occurs upon					PI3-kinase	GP	inhibiton of			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_14_2830_s_161	15241468	( B) Endogenous FoxO3a binds to the  cyclin D2 promoter upon inhibition of PI3-kinase.	bind
347	1	1101	7	10	NULL	0	NULL	FoxO3a	GP	endogenous 	binds to					cyclin D2 	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_embo_23_14_2830_s_161	15241468	( B) Endogenous FoxO3a binds to the  cyclin D2 promoter upon inhibition of PI3-kinase.	bind
350	2	1101	7	10	NULL	0	NULL	statement 1	Process		occurs upon 					PI3-kinase	GP	inhibition of			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_14_2830_s_161	15241468	( B) Endogenous FoxO3a binds to the  cyclin D2 promoter upon inhibition of PI3-kinase.	bind
863	1	1102	5	10	NULL	0	NULL	MLL	GP	endogenous	bind					CDKN1B	GP			promoter	NULL	MV4 - 11 cells	NULL	NULL	NULL	NULL	gw70_pnas_102_39_14028_s_223	16169901	( B) Endogenous MLL/MLL-AF4 binds to the  CDKN1B promoter in MV4 - 11 and RS4;11 cells.	bind
47877	2	1102	5	10	NULL	0	NULL	MLL-AF4	GP	endogenous	bind					CDKN1B	GP			promoter	NULL	MV4 - 11 cells	NULL	NULL	NULL	NULL	gw70_pnas_102_39_14028_s_223	16169901	( B) Endogenous MLL/MLL-AF4 binds to the  CDKN1B promoter in MV4 - 11 and RS4;11 cells.	bind
47878	3	1102	5	10	NULL	0	NULL	MLL	GP	endogenous	bind					CDKN1B	GP			promoter	NULL	RS4;11 cells	NULL	NULL	NULL	NULL	gw70_pnas_102_39_14028_s_223	16169901	( B) Endogenous MLL/MLL-AF4 binds to the  CDKN1B promoter in MV4 - 11 and RS4;11 cells.	bind
47879	4	1102	5	10	NULL	0	NULL	MLL-AF4	GP	endogenous	bind					CDKN1B	GP			promoter	NULL	RS4;11 cells	NULL	NULL	NULL	NULL	gw70_pnas_102_39_14028_s_223	16169901	( B) Endogenous MLL/MLL-AF4 binds to the  CDKN1B promoter in MV4 - 11 and RS4;11 cells.	bind
362	1	1102	7	10	NULL	0	NULL	MLL	GP	endogenous	bind					CDKN1B	GP			promoter	NULL	MV4 - 11 cells	NULL	NULL	NULL	NULL	gw70_pnas_102_39_14028_s_223	16169901	( B) Endogenous MLL/MLL-AF4 binds to the  CDKN1B promoter in MV4 - 11 and RS4;11 cells.	bind
365	2	1102	7	10	NULL	0	NULL	MLL-AF4 	GP	endogenous	bind					CDKN1B	GP			promoter	NULL	MV4 - 11 cells	NULL	NULL	NULL	NULL	gw70_pnas_102_39_14028_s_223	16169901	( B) Endogenous MLL/MLL-AF4 binds to the  CDKN1B promoter in MV4 - 11 and RS4;11 cells.	bind
369	3	1102	7	10	NULL	0	NULL	MLL	GP	endogenous	bind					CDKN1B	GP			promoter	NULL	RS4;11 cells	NULL	NULL	NULL	NULL	gw70_pnas_102_39_14028_s_223	16169901	( B) Endogenous MLL/MLL-AF4 binds to the  CDKN1B promoter in MV4 - 11 and RS4;11 cells.	bind
370	4	1102	7	10	NULL	0	NULL	MLL-AF4 	GP	endogenous	bind					CDKN1B	GP			promoter	NULL	RS4;11 cells	NULL	NULL	NULL	NULL	gw70_pnas_102_39_14028_s_223	16169901	( B) Endogenous MLL/MLL-AF4 binds to the  CDKN1B promoter in MV4 - 11 and RS4;11 cells.	bind
864	1	1103	5	10	NULL	0	NULL	p53beta	GP	endogenous	bind		differentially							p53-responsive promoter	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_18_2122_s_284	16131611	( B) Endogenous p53beta binds differentially to the p53-responsive promoter.	bind
375	1	1103	7	10	NULL	0	NULL	 p53beta 	GP	endogenous\t	bind		 differentially			 				p53-responsive promoter	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_18_2122_s_284	16131611	( B) Endogenous p53beta binds differentially to the p53-responsive promoter.	bind
865	1	1104	5	10	NULL	0	NULL	RASSF1C	GP	endogenous	bind					Daxx	GP	endogenous			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_14_3286_s_86	16810318	( B) Endogenous RASSF1C binds endogenous Daxx.	bind
376	1	1104	7	10	NULL	0	NULL	RASSF1C	GP	endogenous	bind					Daxx	GP	endogenous			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_14_3286_s_86	16810318	( B) Endogenous RASSF1C binds endogenous Daxx.	bind
866	1	1107	5	10	NULL	0	NULL	Yeast	Organism		express					ETR1	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw60_science_283_5404_996_s_72	9974395	( B) Ethylene binding by yeast expressing wild-type and mutant forms of ETR1.	bind
867	2	1107	5	10	NULL	0	NULL	statement 1	Process		bind					Ethylene	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_283_5404_996_s_72	9974395	( B) Ethylene binding by yeast expressing wild-type and mutant forms of ETR1.	bind
48717	3	1107	5	10	NULL	0	NULL	Yeast	Organism		expresses					ETR1	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_science_283_5404_996_s_72	9974395	( B) Ethylene binding by yeast expressing wild-type and mutant forms of ETR1.	bind
48718	4	1107	5	10	NULL	0	NULL	statement 3	Process		bind					Ethylene	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_283_5404_996_s_72	9974395	( B) Ethylene binding by yeast expressing wild-type and mutant forms of ETR1.	bind
377	1	1107	7	10	NULL	0	NULL	Yeast	Organism		expresses					ETR1	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw60_science_283_5404_996_s_72	9974395	( B) Ethylene binding by yeast expressing wild-type and mutant forms of ETR1.	bind
378	2	1107	7	10	NULL	0	NULL	statement 1	Process		bind					Ethylene 	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_283_5404_996_s_72	9974395	( B) Ethylene binding by yeast expressing wild-type and mutant forms of ETR1.	bind
48719	3	1107	7	10	NULL	0	NULL	Yeast	Organism		expresses					ETR1	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_science_283_5404_996_s_72	9974395	( B) Ethylene binding by yeast expressing wild-type and mutant forms of ETR1.	bind
48720	4	1107	7	10	NULL	0	NULL	statement 3	Process		bind					Ethylene	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_283_5404_996_s_72	9974395	( B) Ethylene binding by yeast expressing wild-type and mutant forms of ETR1.	bind
868	1	1110	5	10	NULL	0	NULL	Sema4D	GP		bind					plexin-B1	GP				NULL	HEK293 cells	NULL	NULL	NULL	NULL	gw60_genesdev_16_7_836_s_74	11937491	( B) Expression of RacL61 enhances the binding of Sema4D to plexin-B1 in HEK293 cells.	bind
869	2	1110	5	10	NULL	0	NULL	RacL61	GP		enhances					statement 1	Process				NULL	HEK293 cells	NULL	NULL	NULL	NULL	gw60_genesdev_16_7_836_s_74	11937491	( B) Expression of RacL61 enhances the binding of Sema4D to plexin-B1 in HEK293 cells.	bind
380	1	1110	7	10	NULL	0	NULL	Sema4D	GP		bind					plexin-B1 	GP				NULL	HEK293 cells	NULL	NULL	NULL	NULL	gw60_genesdev_16_7_836_s_74	11937491	( B) Expression of RacL61 enhances the binding of Sema4D to plexin-B1 in HEK293 cells.	bind
382	2	1110	7	10	NULL	0	NULL	RacL61	GP		enhances 					statement 1	Process				NULL	HEK293 cells	NULL	NULL	NULL	NULL	gw60_genesdev_16_7_836_s_74	11937491	( B) Expression of RacL61 enhances the binding of Sema4D to plexin-B1 in HEK293 cells.	bind
870	1	1112	5	10	NULL	0	NULL	YY1	GP		bind		female-specific			Xist cluster	GP				NULL		NULL	NULL	NULL	NULL	gw70_genomeres_16_7_901_s_122	16760423	( B) Female-specific binding of YY1 to the  Xist cluster.	bind
399	1	1112	7	10	NULL	0	NULL	YY1 	GP	 	bind		Female-specific			Xist cluster	GP				NULL		NULL	NULL	NULL	NULL	gw70_genomeres_16_7_901_s_122	16760423	( B) Female-specific binding of YY1 to the  Xist cluster.	bind
873	1	1113	5	10	NULL	0	NULL	SARS-CoV S1180 protein	GP	soluble	bind					CHO cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_44_15748_s_121	15496474	( B) Flow cytometric analysis of soluble SARS-CoV S1180 protein binding to CHO ( Upper) and clone 2.27 ( Lower) cells.	bind
2435	2	1113	5	10	NULL	0	NULL	SARS-CoV S1180 protein	GP	soluble	bind					clone 2.27 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_44_15748_s_121	15496474	( B) Flow cytometric analysis of soluble SARS-CoV S1180 protein binding to CHO ( Upper) and clone 2.27 ( Lower) cells.	bind
404	1	1113	7	10	NULL	0	NULL	SARS-CoV S1180 protein 	GP	soluble	bind					CHO cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_44_15748_s_121	15496474	( B) Flow cytometric analysis of soluble SARS-CoV S1180 protein binding to CHO ( Upper) and clone 2.27 ( Lower) cells.	bind
407	2	1113	7	10	NULL	0	NULL	SARS-CoV S1180 protein 	GP	soluble	bind					clone 2.27 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_44_15748_s_121	15496474	( B) Flow cytometric analysis of soluble SARS-CoV S1180 protein binding to CHO ( Upper) and clone 2.27 ( Lower) cells.	bind
874	1	1114	5	10	NULL	0	NULL	DM	Chemical		bind					apoRfBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_21_11873_s_156	11592998	( B) Fluorescence decays (610 nm) of DM (50 mum) bound to the apoRfBP (400 muM) with a series of concentrations of Gdn.HCl, from 0 M to [[ 2 M.                    To ]] further characterize these "`free"' DM molecules, we measured the time-resolved anisotropy, as shown in Fig.  6 A Inset.	bind
449	1	1114	7	10	NULL	0	NULL	DM	Chemical		binds					 apoRfBP 	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_21_11873_s_156	11592998	( B) Fluorescence decays (610 nm) of DM (50 mum) bound to the apoRfBP (400 muM) with a series of concentrations of Gdn.HCl, from 0 M to [[ 2 M.                    To ]] further characterize these "`free"' DM molecules, we measured the time-resolved anisotropy, as shown in Fig.  6 A Inset.	bind
2436	1	1115	5	10	NULL	0	NULL	four nucleotide	NucleicAcid	substitution of	reduce		significantly			MBNL1	GP	binding of;; recombinant			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_15_3103_s_109	15257297	( B) Four nucleotide substitutions significantly reduce binding of recombinant MBNL1  detected by UV crosslinking.	bind
451	1	1115	7	10	NULL	0	NULL	Four nucleotide	NucleicAcid	substitution of	reduce 		significantly			MBNL1	GP	binding of;; recombinant			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_15_3103_s_109	15257297	( B) Four nucleotide substitutions significantly reduce binding of recombinant MBNL1  detected by UV crosslinking.	bind
878	2	1116	5	10	NULL	0	NULL	Rev14	GP		bind		specifically			RRE IIB RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_8_4247_s_131	9539722	( B) Fourteen arginines (Arg14) or a 14-amino acid Rev peptide (Rev14 corresponds to residues 34-47 of Rev, with Trp-45 Arg and Glu-47 Arg substitutions, and specifically binds RRE IIB RNA; ref.  24) were fused to the HIV Tat activation domain (residues 1-49) in the context of surrounding alanines as shown.	bind
61090	1	1116	5	10	NULL	0	NULL	Arg14	AminoAcid		bind		specifically			RRE IIB RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_8_4247_s_131	9539722	( B) Fourteen arginines (Arg14) or a 14-amino acid Rev peptide (Rev14 corresponds to residues 34-47 of Rev, with Trp-45 Arg and Glu-47 Arg substitutions, and specifically binds RRE IIB RNA; ref.  24) were fused to the HIV Tat activation domain (residues 1-49) in the context of surrounding alanines as shown.	bind
61091	3	1116	5	10	NULL	0	NULL	Arg14	AminoAcid		is					Fourteen arginines	AminoAcid				NULL		0	NULL	NULL	NULL	gw60_pnas_95_8_4247_s_131	9539722	( B) Fourteen arginines (Arg14) or a 14-amino acid Rev peptide (Rev14 corresponds to residues 34-47 of Rev, with Trp-45 Arg and Glu-47 Arg substitutions, and specifically binds RRE IIB RNA; ref.  24) were fused to the HIV Tat activation domain (residues 1-49) in the context of surrounding alanines as shown.	bind
61092	4	1116	5	10	NULL	0	NULL	Rev14	GP		is					14-amino acid Rev peptide	GP		residues 34-47, with Trp-45 Arg and Glu-47 Arg substitutions		NULL		0	NULL	NULL	NULL	gw60_pnas_95_8_4247_s_131	9539722	( B) Fourteen arginines (Arg14) or a 14-amino acid Rev peptide (Rev14 corresponds to residues 34-47 of Rev, with Trp-45 Arg and Glu-47 Arg substitutions, and specifically binds RRE IIB RNA; ref.  24) were fused to the HIV Tat activation domain (residues 1-49) in the context of surrounding alanines as shown.	bind
454	1	1116	7	10	NULL	0	NULL	Arg14	AminoAcid		bind		specifically			RRE IIB RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_8_4247_s_131	9539722	( B) Fourteen arginines (Arg14) or a 14-amino acid Rev peptide (Rev14 corresponds to residues 34-47 of Rev, with Trp-45 Arg and Glu-47 Arg substitutions, and specifically binds RRE IIB RNA; ref.  24) were fused to the HIV Tat activation domain (residues 1-49) in the context of surrounding alanines as shown.	bind
534	2	1116	7	10	NULL	0	NULL	 Rev14	GP		bind		specifically			RRE IIB RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_8_4247_s_131	9539722	( B) Fourteen arginines (Arg14) or a 14-amino acid Rev peptide (Rev14 corresponds to residues 34-47 of Rev, with Trp-45 Arg and Glu-47 Arg substitutions, and specifically binds RRE IIB RNA; ref.  24) were fused to the HIV Tat activation domain (residues 1-49) in the context of surrounding alanines as shown.	bind
536	3	1116	7	10	NULL	0	NULL	Arg14	AminoAcid		is					Fourteen arginines	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_8_4247_s_131	9539722	( B) Fourteen arginines (Arg14) or a 14-amino acid Rev peptide (Rev14 corresponds to residues 34-47 of Rev, with Trp-45 Arg and Glu-47 Arg substitutions, and specifically binds RRE IIB RNA; ref.  24) were fused to the HIV Tat activation domain (residues 1-49) in the context of surrounding alanines as shown.	bind
537	4	1116	7	10	NULL	0	NULL	Rev14	GP		is					14-amino acid Rev peptide	GP		residues 34-47, with Trp-45 Arg and Glu-47 Arg substitutions		NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_8_4247_s_131	9539722	( B) Fourteen arginines (Arg14) or a 14-amino acid Rev peptide (Rev14 corresponds to residues 34-47 of Rev, with Trp-45 Arg and Glu-47 Arg substitutions, and specifically binds RRE IIB RNA; ref.  24) were fused to the HIV Tat activation domain (residues 1-49) in the context of surrounding alanines as shown.	bind
880	1	1117	5	10	NULL	0	NULL	Sug1/Rpt6 protein	GP		bind					GAL1-10	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_science_296_5567_548_s_35	11964484	( B) Gal4 dependence of Sug1/Rpt6 protein binding to the  GAL1-10 promoter.	bind
881	2	1117	5	10	NULL	0	NULL	statement 1	Process		is dependent on					Gal4	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_296_5567_548_s_35	11964484	( B) Gal4 dependence of Sug1/Rpt6 protein binding to the  GAL1-10 promoter.	bind
541	1	1117	7	10	NULL	0	NULL	Sug1/Rpt6 protein	GP		bind					GAL1-10 	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_science_296_5567_548_s_35	11964484	( B) Gal4 dependence of Sug1/Rpt6 protein binding to the  GAL1-10 promoter.	bind
543	2	1117	7	10	NULL	0	NULL	statement 1	Process		is dependent on					Gal4	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_296_5567_548_s_35	11964484	( B) Gal4 dependence of Sug1/Rpt6 protein binding to the  GAL1-10 promoter.	bind
882	1	1118	5	10	NULL	0	NULL	GATA	GP		bind					PPARgamma2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_science_290_5489_134_s_71	11021798	( B) GATA binding to PPARgamma2 promoter determined by DNase I footprinting analysis.	bind
545	1	1118	7	10	NULL	0	NULL	GATA 	GP		bind					PPARgamma2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_science_290_5489_134_s_71	11021798	( B) GATA binding to PPARgamma2 promoter determined by DNase I footprinting analysis.	bind
883	1	1119	5	10	NULL	0	NULL	GDP-Gpa2	GP		bind					adenylate cyclase	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_17_6108_s_197	15831585	( B) GDP-Gpa2 binding to adenylate cyclase facilitates binding of the activated GTP-Gpa2  to both the N-terminal domain and to a site within the catalytic domain that stimulates  adenylate cyclase activity.	bind
884	2	1119	5	10	NULL	0	NULL	GTP-Gpa2	GP	activated	bind					adenylate cyclase	GP		N-terminal domain		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_17_6108_s_197	15831585	( B) GDP-Gpa2 binding to adenylate cyclase facilitates binding of the activated GTP-Gpa2  to both the N-terminal domain and to a site within the catalytic domain that stimulates  adenylate cyclase activity.	bind
885	3	1119	5	10	NULL	0	NULL	GTP-Gpa2	GP	activated	bind					adenylate cyclase	GP		a site within catalytic domain		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_17_6108_s_197	15831585	( B) GDP-Gpa2 binding to adenylate cyclase facilitates binding of the activated GTP-Gpa2  to both the N-terminal domain and to a site within the catalytic domain that stimulates  adenylate cyclase activity.	bind
886	4	1119	5	10	NULL	0	NULL	statement 1	Process		facilitate					statement 2 	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_17_6108_s_197	15831585	( B) GDP-Gpa2 binding to adenylate cyclase facilitates binding of the activated GTP-Gpa2  to both the N-terminal domain and to a site within the catalytic domain that stimulates  adenylate cyclase activity.	bind
47880	5	1119	5	10	NULL	0	NULL	statement 1	Process		facilitate					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_17_6108_s_197	15831585	( B) GDP-Gpa2 binding to adenylate cyclase facilitates binding of the activated GTP-Gpa2  to both the N-terminal domain and to a site within the catalytic domain that stimulates  adenylate cyclase activity.	bind
547	1	1119	7	10	NULL	0	NULL	GDP-Gpa2	GP		bind					adenylate cyclase 	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_17_6108_s_197	15831585	( B) GDP-Gpa2 binding to adenylate cyclase facilitates binding of the activated GTP-Gpa2  to both the N-terminal domain and to a site within the catalytic domain that stimulates  adenylate cyclase activity.	bind
549	2	1119	7	10	NULL	0	NULL	GTP-Gpa2	GP	activated	bind					adenylate cyclase	GP		N-terminal domain 		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_17_6108_s_197	15831585	( B) GDP-Gpa2 binding to adenylate cyclase facilitates binding of the activated GTP-Gpa2  to both the N-terminal domain and to a site within the catalytic domain that stimulates  adenylate cyclase activity.	bind
550	3	1119	7	10	NULL	0	NULL	GTP-Gpa2	GP	activated	binds to					adenylate cyclase	GP		 site within the catalytic domain		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_17_6108_s_197	15831585	( B) GDP-Gpa2 binding to adenylate cyclase facilitates binding of the activated GTP-Gpa2  to both the N-terminal domain and to a site within the catalytic domain that stimulates  adenylate cyclase activity.	bind
1168	4	1119	7	10	NULL	0	NULL	statement 1	Process		facilitate					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_17_6108_s_197	15831585	( B) GDP-Gpa2 binding to adenylate cyclase facilitates binding of the activated GTP-Gpa2  to both the N-terminal domain and to a site within the catalytic domain that stimulates  adenylate cyclase activity.	bind
1171	5	1119	7	10	NULL	0	NULL	statement 1	Process		facilitate					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_17_6108_s_197	15831585	( B) GDP-Gpa2 binding to adenylate cyclase facilitates binding of the activated GTP-Gpa2  to both the N-terminal domain and to a site within the catalytic domain that stimulates  adenylate cyclase activity.	bind
887	1	1120	5	10	NULL	0	NULL	AEF-1 protein	GP		bind					Adh	GP			proximal promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_17_4_1076_s_53	9463385	( B) Gel mobility shift assay showing the binding of AEF-1 protein to the  Adh proximal promoter but not to the distal promoter.	bind
888	2	1120	5	10	NULL	0	NULL	AEF-1 protein	GP		does not bind					Adh	GP			distal promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_17_4_1076_s_53	9463385	( B) Gel mobility shift assay showing the binding of AEF-1 protein to the  Adh proximal promoter but not to the distal promoter.	bind
551	1	1120	7	10	NULL	0	NULL	AEF-1protein	GP		binds to					 Adh 	GP			proximal promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_17_4_1076_s_53	9463385	( B) Gel mobility shift assay showing the binding of AEF-1 protein to the  Adh proximal promoter but not to the distal promoter.	bind
552	2	1120	7	10	NULL	0	NULL	AEF-1 protein 	GP		does not bind					Adh	GP			distal promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_17_4_1076_s_53	9463385	( B) Gel mobility shift assay showing the binding of AEF-1 protein to the  Adh proximal promoter but not to the distal promoter.	bind
889	1	1121	5	10	NULL	0	NULL	MEF2A proteins	GP	 in vitro translated	bind									N10 site	NULL		NULL	NULL	NULL	NULL	gw60_embo_19_11_2615_s_117	10835359	( B) Gel retardation analysis of equimolar concentrations of  in vitro translated MEF2A proteins bound to the N10 site (central motif CTATTTATAG; Sharrocks  et al., 1993a).	bind
47881	2	1121	5	10	NULL	0	NULL	N10 site	GP		is									central motif CTATTTATAG	NULL		NULL	NULL	NULL	NULL	gw60_embo_19_11_2615_s_117	10835359	( B) Gel retardation analysis of equimolar concentrations of  in vitro translated MEF2A proteins bound to the N10 site (central motif CTATTTATAG; Sharrocks  et al., 1993a).	bind
553	1	1121	7	10	NULL	0	NULL	MEF2A proteins 	GP	in vitro translated 	bind to									N10 site 	NULL		NULL	NULL	NULL	NULL	gw60_embo_19_11_2615_s_117	10835359	( B) Gel retardation analysis of equimolar concentrations of  in vitro translated MEF2A proteins bound to the N10 site (central motif CTATTTATAG; Sharrocks  et al., 1993a).	bind
47882	2	1121	7	10	NULL	0	NULL	N10 site	GP		is									central motif CTATTTATAG	NULL		NULL	NULL	NULL	NULL	gw60_embo_19_11_2615_s_117	10835359	( B) Gel retardation analysis of equimolar concentrations of  in vitro translated MEF2A proteins bound to the N10 site (central motif CTATTTATAG; Sharrocks  et al., 1993a).	bind
890	1	1122	5	10	NULL	0	NULL	Taz1p	GP	in vitro translated	bind									140 bp telomeric fragment	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_2_527_s_46	10606652	( B) Gel retardation assay showing  in vitro translated (IVT) Taz1p binding to the 140 bp telomeric fragment.	bind
554	1	1122	7	10	NULL	0	NULL	Taz1p	GP	 in vitro translated 	bind									140 bp telomeric fragment	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_2_527_s_46	10606652	( B) Gel retardation assay showing  in vitro translated (IVT) Taz1p binding to the 140 bp telomeric fragment.	bind
891	1	1123	5	10	NULL	0	NULL	R2 protein	GP	full-length	bind					DNA substrates	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_20_6461_s_53	16284201	( B) Gel shifts of the full-length R2 protein bound to mutant DNA substrates at low (36  fmol) and high (360 fmol) protein concentrations in the absence of dNTPs.	bind
555	1	1123	7	10	NULL	0	NULL	 R2 protein 	GP	full-length 	bind					DNA substrates 	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_20_6461_s_53	16284201	( B) Gel shifts of the full-length R2 protein bound to mutant DNA substrates at low (36  fmol) and high (360 fmol) protein concentrations in the absence of dNTPs.	bind
892	1	1124	5	10	NULL	0	NULL	ChREBP	GP		bind to					lipogenic gene	GP			ChRE in promoter of	NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_44_15597_s_132	15496471	( B) Gel-shift analysis of ChREBP bound to the ChREs of lipogenic gene promoters after  immunoreaction with ChREBP antibodies.	bind
557	1	1124	7	10	NULL	0	NULL	ChREBP	GP		bind to					lipogenic gene	GP			ChRE of promoter	NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_44_15597_s_132	15496471	( B) Gel-shift analysis of ChREBP bound to the ChREs of lipogenic gene promoters after  immunoreaction with ChREBP antibodies.	bind
893	1	1125	5	10	NULL	0	NULL	E-cadherin	GP	glycosylated	bind					beta-catenin	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_21_5999_s_219	11689440	( B) Glycosylated E-cadherin binds beta- and gamma-catenin but not p120-catenin.	bind
894	2	1125	5	10	NULL	0	NULL	E-cadherin	GP	glycosylated	bind					gamma-catenin	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_21_5999_s_219	11689440	( B) Glycosylated E-cadherin binds beta- and gamma-catenin but not p120-catenin.	bind
895	3	1125	5	10	NULL	0	NULL	E-cadherin	GP	glycosylated	does not bind					p120-catenin	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_21_5999_s_219	11689440	( B) Glycosylated E-cadherin binds beta- and gamma-catenin but not p120-catenin.	bind
559	1	1125	7	10	NULL	0	NULL	E-cadherin 	GP	Glycosylated	bind					beta-catenin	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_21_5999_s_219	11689440	( B) Glycosylated E-cadherin binds beta- and gamma-catenin but not p120-catenin.	bind
560	2	1125	7	10	NULL	0	NULL	E-cadherin 	GP	Glycosylated	bind					gamma-catenin 	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_21_5999_s_219	11689440	( B) Glycosylated E-cadherin binds beta- and gamma-catenin but not p120-catenin.	bind
561	3	1125	7	10	NULL	0	NULL	E-cadherin 	GP	Glycosylated	does not bind					p120-catenin	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_21_5999_s_219	11689440	( B) Glycosylated E-cadherin binds beta- and gamma-catenin but not p120-catenin.	bind
901	1	1127	5	10	NULL	0	NULL	ScMre11p	GP		bind					G4 DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_15_4692_s_146	16116037	( B) Graph showing binding of ScMre11p to G4 DNA.	bind
597	1	1127	7	10	NULL	0	NULL	ScMre11p	GP		bind					G4 DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_15_4692_s_146	16116037	( B) Graph showing binding of ScMre11p to G4 DNA.	bind
902	1	1128	5	10	NULL	0	NULL	RNase III	GP		bind					R1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_9_2381_s_306	12711683	( B) Graphic presentation of the effect of the db17 mutation on RNase III binding to  R1.	bind
47890	2	1128	5	10	NULL	0	NULL	db17	NucleicAcid	mutant	effects					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_9_2381_s_306	12711683	( B) Graphic presentation of the effect of the db17 mutation on RNase III binding to  R1.	bind
598	1	1128	7	10	NULL	0	NULL	RNase III 	GP		bind					R1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_9_2381_s_306	12711683	( B) Graphic presentation of the effect of the db17 mutation on RNase III binding to  R1.	bind
599	2	1128	7	10	NULL	0	NULL	db17 	NucleicAcid	mutant	effects					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_9_2381_s_306	12711683	( B) Graphic presentation of the effect of the db17 mutation on RNase III binding to  R1.	bind
903	1	1132	5	10	NULL	0	NULL	GST-AKIP	GP		bind		directly							C subunit	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_2_349_s_158	15630084	( B) GST pull down showed direct binding of the C subunit with GST-AKIP* as analyzed by SDS/PAGE.	bind
600	1	1132	7	10	NULL	0	NULL				bind		directly	C subunit 		GST-AKIP	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_2_349_s_158	15630084	( B) GST pull down showed direct binding of the C subunit with GST-AKIP* as analyzed by SDS/PAGE.	bind
904	1	1133	5	10	NULL	0	NULL	BRCA2	GP		bind					RAD51	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_pnas_95_9_5287_s_121	9560268	( B) GST pull-down assay for the   in vitro binding of BRCA2 to RAD51.	bind
601	1	1133	7	10	NULL	0	NULL	BRCA2	GP		bind					RAD51	GP				NULL	 in vitro 	NULL	NULL	NULL	NULL	gw60_pnas_95_9_5287_s_121	9560268	( B) GST pull-down assay for the   in vitro binding of BRCA2 to RAD51.	bind
905	1	1134	5	10	NULL	0	NULL	Elk	GP		bind			1-93		Elk-1	GP	non-phosphorylated;; GST fusion protein	C-terminal domain		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_20_5666_s_140	10523309	( B) GST pull-down assay of binding of Elk1-93 and Elk1-168 to GST fusion proteins containing the non-phosphorylated and phosphorylated C-terminal domain of Elk-1.	bind
906	2	1134	5	10	NULL	0	NULL	Elk	GP		bind			1-93		Elk-1	GP	phosphorylated;; GST fusion protein	C-terminal domain		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_20_5666_s_140	10523309	( B) GST pull-down assay of binding of Elk1-93 and Elk1-168 to GST fusion proteins containing the non-phosphorylated and phosphorylated C-terminal domain of Elk-1.	bind
907	3	1134	5	10	NULL	0	NULL	Elk	GP		bind			1-168		Elk-1	GP	non-phosphorylated;; GST fusion protein	C-terminal domain		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_20_5666_s_140	10523309	( B) GST pull-down assay of binding of Elk1-93 and Elk1-168 to GST fusion proteins containing the non-phosphorylated and phosphorylated C-terminal domain of Elk-1.	bind
908	4	1134	5	10	NULL	0	NULL	Elk	GP		bind			1-168		Elk-1	GP	phosphorylated;; GST fusion protein	C-terminal domain		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_20_5666_s_140	10523309	( B) GST pull-down assay of binding of Elk1-93 and Elk1-168 to GST fusion proteins containing the non-phosphorylated and phosphorylated C-terminal domain of Elk-1.	bind
602	1	1134	7	10	NULL	0	NULL	Elk	GP		bind			1-93 		Elk-1	GP	GST fusion proteins;; non-phosphorylated	C-terminal domain 		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_20_5666_s_140	10523309	( B) GST pull-down assay of binding of Elk1-93 and Elk1-168 to GST fusion proteins containing the non-phosphorylated and phosphorylated C-terminal domain of Elk-1.	bind
603	2	1134	7	10	NULL	0	NULL	Elk	GP		bind			1-93		Elk-1	GP	GST fusion proteins;; phosphorylated	C-terminal domain 		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_20_5666_s_140	10523309	( B) GST pull-down assay of binding of Elk1-93 and Elk1-168 to GST fusion proteins containing the non-phosphorylated and phosphorylated C-terminal domain of Elk-1.	bind
604	3	1134	7	10	NULL	0	NULL	Elk	GP		bind			1-168 		Elk-1	GP	GST fusion proteins;; non-phosphorylated	C-terminal domain 		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_20_5666_s_140	10523309	( B) GST pull-down assay of binding of Elk1-93 and Elk1-168 to GST fusion proteins containing the non-phosphorylated and phosphorylated C-terminal domain of Elk-1.	bind
605	4	1134	7	10	NULL	0	NULL	Elk	GP		bind			1-168 		Elk-1	GP	GST fusion protein;; phosphorylated 	C-terminal domain 		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_20_5666_s_140	10523309	( B) GST pull-down assay of binding of Elk1-93 and Elk1-168 to GST fusion proteins containing the non-phosphorylated and phosphorylated C-terminal domain of Elk-1.	bind
909	1	1135	5	10	NULL	0	NULL	PC	GP		bind					GST-C127/203	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_11_2873_s_169	12771214	( B) GST pull-down experiments: binding of PC, PH and SCM to GST, GST-C127/203 and GST-Corto.	bind
910	2	1135	5	10	NULL	0	NULL	PH	GP		bind					GST-C127/203	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_11_2873_s_169	12771214	( B) GST pull-down experiments: binding of PC, PH and SCM to GST, GST-C127/203 and GST-Corto.	bind
911	3	1135	5	10	NULL	0	NULL	SCM	GP		bind					GST-C127/203	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_11_2873_s_169	12771214	( B) GST pull-down experiments: binding of PC, PH and SCM to GST, GST-C127/203 and GST-Corto.	bind
912	4	1135	5	10	NULL	0	NULL	PC	GP		bind					GST-Corto	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_11_2873_s_169	12771214	( B) GST pull-down experiments: binding of PC, PH and SCM to GST, GST-C127/203 and GST-Corto.	bind
913	5	1135	5	10	NULL	0	NULL	PH	GP		bind					GST-Corto	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_11_2873_s_169	12771214	( B) GST pull-down experiments: binding of PC, PH and SCM to GST, GST-C127/203 and GST-Corto.	bind
914	6	1135	5	10	NULL	0	NULL	SCM	GP		bind					GST-Corto	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_11_2873_s_169	12771214	( B) GST pull-down experiments: binding of PC, PH and SCM to GST, GST-C127/203 and GST-Corto.	bind
48843	7	1135	5	10	NULL	0	NULL	PC	GP		bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_11_2873_s_169	12771214	( B) GST pull-down experiments: binding of PC, PH and SCM to GST, GST-C127/203 and GST-Corto.	bind
48844	8	1135	5	10	NULL	0	NULL	PH	GP		bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_11_2873_s_169	12771214	( B) GST pull-down experiments: binding of PC, PH and SCM to GST, GST-C127/203 and GST-Corto.	bind
48845	9	1135	5	10	NULL	0	NULL	SCM	GP		bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_11_2873_s_169	12771214	( B) GST pull-down experiments: binding of PC, PH and SCM to GST, GST-C127/203 and GST-Corto.	bind
606	1	1135	7	10	NULL	0	NULL	PC	GP		bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_11_2873_s_169	12771214	( B) GST pull-down experiments: binding of PC, PH and SCM to GST, GST-C127/203 and GST-Corto.	bind
607	2	1135	7	10	NULL	0	NULL	PC	GP		bind					GST-C127/203	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_11_2873_s_169	12771214	( B) GST pull-down experiments: binding of PC, PH and SCM to GST, GST-C127/203 and GST-Corto.	bind
608	3	1135	7	10	NULL	0	NULL	PC	GP		bind					GST-Corto	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_11_2873_s_169	12771214	( B) GST pull-down experiments: binding of PC, PH and SCM to GST, GST-C127/203 and GST-Corto.	bind
640	4	1135	7	10	NULL	0	NULL	PH 	GP		bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_11_2873_s_169	12771214	( B) GST pull-down experiments: binding of PC, PH and SCM to GST, GST-C127/203 and GST-Corto.	bind
641	5	1135	7	10	NULL	0	NULL	PH	GP		bind					GST-C127/203	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_11_2873_s_169	12771214	( B) GST pull-down experiments: binding of PC, PH and SCM to GST, GST-C127/203 and GST-Corto.	bind
642	6	1135	7	10	NULL	0	NULL	PH	GP		bind					GST-Corto	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_11_2873_s_169	12771214	( B) GST pull-down experiments: binding of PC, PH and SCM to GST, GST-C127/203 and GST-Corto.	bind
643	7	1135	7	10	NULL	0	NULL	SCM	GP		bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_11_2873_s_169	12771214	( B) GST pull-down experiments: binding of PC, PH and SCM to GST, GST-C127/203 and GST-Corto.	bind
644	8	1135	7	10	NULL	0	NULL	SCM	GP		bind					GST-C127/203	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_11_2873_s_169	12771214	( B) GST pull-down experiments: binding of PC, PH and SCM to GST, GST-C127/203 and GST-Corto.	bind
645	9	1135	7	10	NULL	0	NULL	SCM	GP		bind					GST-Corto	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_11_2873_s_169	12771214	( B) GST pull-down experiments: binding of PC, PH and SCM to GST, GST-C127/203 and GST-Corto.	bind
915	1	1136	5	10	NULL	0	NULL	Molt-4 protein	GP		bind					TdT constructs	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_19_10746_s_86	12960389	( B) GST pull-down of Molt-4 and Nalm-6 proteins binding to TdT constructs.	bind
916	2	1136	5	10	NULL	0	NULL	Nalm-6 protein	GP		bind					TdT constructs	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_19_10746_s_86	12960389	( B) GST pull-down of Molt-4 and Nalm-6 proteins binding to TdT constructs.	bind
646	1	1136	7	10	NULL	0	NULL	Molt-4 protein	GP		bind					TdT constructs	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_19_10746_s_86	12960389	( B) GST pull-down of Molt-4 and Nalm-6 proteins binding to TdT constructs.	bind
647	2	1136	7	10	NULL	0	NULL	Nalm-6 protein	GP		bind					TdT constructs	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_19_10746_s_86	12960389	( B) GST pull-down of Molt-4 and Nalm-6 proteins binding to TdT constructs.	bind
917	1	1138	5	10	NULL	0	NULL	GST-(CTLA-4)3	GP	fusion protein	bind					TCRzeta	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_282_5397_2263_s_71	9856951	( B) GST-(CTLA-4)3 fusion protein binds TCRzeta.	bind
648	1	1138	7	10	NULL	0	NULL	GST-(CTLA-4)3	GP	fusion protein	binds					TCRzeta	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_282_5397_2263_s_71	9856951	( B) GST-(CTLA-4)3 fusion protein binds TCRzeta.	bind
918	1	1139	5	10	NULL	0	NULL	GST-Rtt106p	GP		bind					CAF-1 complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_38_13410_s_138	16157874	( B) GST-Rtt106p bound to the CAF-1 complex.	bind
649	1	1139	7	10	NULL	0	NULL	GST-Rtt106p	GP		bind					CAF-1 complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_38_13410_s_138	16157874	( B) GST-Rtt106p bound to the CAF-1 complex.	bind
919	1	1141	5	10	NULL	0	NULL	H-Ras	GP		bind					PLCepsilon	GP		RA domains		NULL		NULL	NULL	NULL	NULL	gw60_embo_20_4_743_s_93	11179219	( B) H-Ras binding to RA domains of PLCepsilon and the RBD of Raf-1.	bind
920	2	1141	5	10	NULL	0	NULL	H-Ras	GP		bind					Raf-1	GP		RBD		NULL		NULL	NULL	NULL	NULL	gw60_embo_20_4_743_s_93	11179219	( B) H-Ras binding to RA domains of PLCepsilon and the RBD of Raf-1.	bind
650	1	1141	7	10	NULL	0	NULL	H-Ras	GP		bind					PLCepsilon	GP		RA domains		NULL		NULL	NULL	NULL	NULL	gw60_embo_20_4_743_s_93	11179219	( B) H-Ras binding to RA domains of PLCepsilon and the RBD of Raf-1.	bind
651	2	1141	7	10	NULL	0	NULL	H-Ras	GP		bind					Raf-1	GP		RBD		NULL		NULL	NULL	NULL	NULL	gw60_embo_20_4_743_s_93	11179219	( B) H-Ras binding to RA domains of PLCepsilon and the RBD of Raf-1.	bind
921	1	1144	5	10	NULL	0	NULL	HetR	GP		bind					hetR 	GP			F hetR-2 of promoter	NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_14_4848_s_152	15051891	( B) HetR binding to the fragment F hetR-2 from the  hetR promoter.	bind
652	1	1144	7	10	NULL	0	NULL	HetR	GP		bind					hetR	GP			F hetR-2 of promoter	NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_14_4848_s_152	15051891	( B) HetR binding to the fragment F hetR-2 from the  hetR promoter.	bind
922	1	1145	5	10	NULL	0	NULL				bind			F302W		iC3b	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_143_6_1523_s_260	9852148	( B) Histograms (mean  plus-or-minus  SEM,  n = 5) showing a selective gain of  binding of F302W to iC3b but  not to NIF, and a selective loss  of binding of T209A to iC3b  but not to NIF.	bind
923	2	1145	5	10	NULL	0	NULL				bind			F302W		NIF	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_143_6_1523_s_260	9852148	( B) Histograms (mean  plus-or-minus  SEM,  n = 5) showing a selective gain of  binding of F302W to iC3b but  not to NIF, and a selective loss  of binding of T209A to iC3b  but not to NIF.	bind
924	3	1145	5	10	NULL	0	NULL				bind			T209A		iC3b	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_143_6_1523_s_260	9852148	( B) Histograms (mean  plus-or-minus  SEM,  n = 5) showing a selective gain of  binding of F302W to iC3b but  not to NIF, and a selective loss  of binding of T209A to iC3b  but not to NIF.	bind
925	4	1145	5	10	NULL	0	NULL				bind			T209A		NIF	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_143_6_1523_s_260	9852148	( B) Histograms (mean  plus-or-minus  SEM,  n = 5) showing a selective gain of  binding of F302W to iC3b but  not to NIF, and a selective loss  of binding of T209A to iC3b  but not to NIF.	bind
668	1	1145	7	10	NULL	0	NULL				bind			F302W		iC3b	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_143_6_1523_s_260	9852148	( B) Histograms (mean  plus-or-minus  SEM,  n = 5) showing a selective gain of  binding of F302W to iC3b but  not to NIF, and a selective loss  of binding of T209A to iC3b  but not to NIF.	bind
670	2	1145	7	10	NULL	0	NULL				bind			F302W		NIF	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_143_6_1523_s_260	9852148	( B) Histograms (mean  plus-or-minus  SEM,  n = 5) showing a selective gain of  binding of F302W to iC3b but  not to NIF, and a selective loss  of binding of T209A to iC3b  but not to NIF.	bind
682	3	1145	7	10	NULL	0	NULL				bind			T209A		iC3b	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_143_6_1523_s_260	9852148	( B) Histograms (mean  plus-or-minus  SEM,  n = 5) showing a selective gain of  binding of F302W to iC3b but  not to NIF, and a selective loss  of binding of T209A to iC3b  but not to NIF.	bind
719	4	1145	7	10	NULL	0	NULL				bind			T209A		NIF	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_143_6_1523_s_260	9852148	( B) Histograms (mean  plus-or-minus  SEM,  n = 5) showing a selective gain of  binding of F302W to iC3b but  not to NIF, and a selective loss  of binding of T209A to iC3b  but not to NIF.	bind
926	1	1146	5	10	NULL	0	NULL	Hog1	GP		bind					STL1	GP			promoter	NULL	cells overexpressing Hot1	NULL	NULL	NULL	NULL	gw60_embo_22_10_2433_s_121	12743037	( B) Hog1 binds to  STL1 promoter upon stress in cells overexpressing Hot1.	bind
2437	2	1146	5	10	NULL	0	NULL	statement 1	Process		occurs upon					 stress	Process				NULL	cells overexpressing Hot1	NULL	NULL	NULL	NULL	gw60_embo_22_10_2433_s_121	12743037	( B) Hog1 binds to  STL1 promoter upon stress in cells overexpressing Hot1.	bind
720	1	1146	7	10	NULL	0	NULL	Hog1	GP		bind					STL1	GP			promoter	NULL	cells overexpressing Hot1	NULL	NULL	NULL	NULL	gw60_embo_22_10_2433_s_121	12743037	( B) Hog1 binds to  STL1 promoter upon stress in cells overexpressing Hot1.	bind
721	2	1146	7	10	NULL	0	NULL	statement 1	Process		occurs upon					 stress	Process				NULL	cells overexpressing Hot1	NULL	NULL	NULL	NULL	gw60_embo_22_10_2433_s_121	12743037	( B) Hog1 binds to  STL1 promoter upon stress in cells overexpressing Hot1.	bind
927	1	1147	5	10	NULL	0	NULL	HCR1	GP		bind			homologous domains		PRT1	GP		RRM		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_20_4_891_s_167	11179233	( B) Homologous domains in HCR1 and TIF32 bind to the PRT1 RRM  in vitro.	bind
928	2	1147	5	10	NULL	0	NULL	TIF32	GP		bind			homologous domains		PRT1	GP		RRM		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_20_4_891_s_167	11179233	( B) Homologous domains in HCR1 and TIF32 bind to the PRT1 RRM  in vitro.	bind
722	1	1147	7	10	NULL	0	NULL	HCR1	GP		bind to			Homologous domain		PRT1	GP		RRM		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_20_4_891_s_167	11179233	( B) Homologous domains in HCR1 and TIF32 bind to the PRT1 RRM  in vitro.	bind
723	2	1147	7	10	NULL	0	NULL	TIF32	GP		bind to			Homologous domain		PRT1	GP		RRM		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_20_4_891_s_167	11179233	( B) Homologous domains in HCR1 and TIF32 bind to the PRT1 RRM  in vitro.	bind
929	1	1148	5	10	NULL	0	NULL	HOS1	GP		bind					ICE1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_103_21_8281_s_96	16702557	( B) HOS1 binds to ICE1  in vitro.	bind
724	1	1148	7	10	NULL	0	NULL	HOS1	GP		bind					ICE1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_103_21_8281_s_96	16702557	( B) HOS1 binds to ICE1  in vitro.	bind
930	2	1149	5	10	NULL	0	NULL	HP1	GP		bind					chromosome 2	Chromosome			rl locus in pericentric region	NULL		NULL	NULL	NULL	NULL	gw70_genomeres_15_9_1265_s_82	16109969	( B) HP1 binding to the  rl locus in the pericentric region of chromosome 2.	bind
725	1	1149	7	10	NULL	0	NULL	HP1	GP		bind					chromosome 2	Chromosome			rl locus in the pericentric region	NULL		NULL	NULL	NULL	NULL	gw70_genomeres_15_9_1265_s_82	16109969	( B) HP1 binding to the  rl locus in the pericentric region of chromosome 2.	bind
931	2	1150	5	10	NULL	0	NULL	HP1beta	GP		bind		directly			Dnmt3a	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_9_2305_s_171	12711675	( B) HP1beta binds directly to Dnmt3a.	bind
726	1	1150	7	10	NULL	0	NULL	HP1beta	GP		bind		direct			Dnmt3a	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_9_2305_s_171	12711675	( B) HP1beta binds directly to Dnmt3a.	bind
932	1	1151	5	10	NULL	0	NULL	GABAAR beta3	GP	human	bind					BTX	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_53	16549768	( b) Human (h) GABAAR beta3 binds BTX, but human GABAAR beta1 does not.	bind
933	2	1151	5	10	NULL	0	NULL	GABAAR beta1	GP	human	does not bind					BTX	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_53	16549768	( b) Human (h) GABAAR beta3 binds BTX, but human GABAAR beta1 does not.	bind
727	1	1151	7	10	NULL	0	NULL	GABAAR beta3	GP	Human	bind					BTX	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_53	16549768	( b) Human (h) GABAAR beta3 binds BTX, but human GABAAR beta1 does not.	bind
728	2	1151	7	10	NULL	0	NULL	GABAAR beta1	GP	Human	does not bind					BTX	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_53	16549768	( b) Human (h) GABAAR beta3 binds BTX, but human GABAAR beta1 does not.	bind
935	1	1152	5	10	NULL	0	NULL	GTP	Chemical		bind					Galpha13	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_280_5372_2109_s_59	9641915	( B) Hydrolysis of GTP bound to Galpha13 ( ) or Galpha12 ( ) was measured at 4 degrees C in the presence of the indicated concentrations of p115 RhoGEF.	bind
936	2	1152	5	10	NULL	0	NULL	GTP	Chemical		bind					Galpha12	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_280_5372_2109_s_59	9641915	( B) Hydrolysis of GTP bound to Galpha13 ( ) or Galpha12 ( ) was measured at 4 degrees C in the presence of the indicated concentrations of p115 RhoGEF.	bind
937	3	1152	5	10	NULL	0	NULL	statement 1	Process		 hydrolyze					p115 RhoGEF	GP	in the presence of			NULL		NULL	NULL	NULL	NULL	gw60_science_280_5372_2109_s_59	9641915	( B) Hydrolysis of GTP bound to Galpha13 ( ) or Galpha12 ( ) was measured at 4 degrees C in the presence of the indicated concentrations of p115 RhoGEF.	bind
938	4	1152	5	10	NULL	0	NULL	statement 2	Process		 hydrolyze					p115 RhoGEF	GP	in the presence of			NULL		NULL	NULL	NULL	NULL	gw60_science_280_5372_2109_s_59	9641915	( B) Hydrolysis of GTP bound to Galpha13 ( ) or Galpha12 ( ) was measured at 4 degrees C in the presence of the indicated concentrations of p115 RhoGEF.	bind
729	1	1152	7	10	NULL	0	NULL	GTP 	Chemical		bind					Galpha13	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_280_5372_2109_s_59	9641915	( B) Hydrolysis of GTP bound to Galpha13 ( ) or Galpha12 ( ) was measured at 4 degrees C in the presence of the indicated concentrations of p115 RhoGEF.	bind
733	3	1152	7	10	NULL	0	NULL	statement 1	Process		 hydrolyze					p115 RhoGEF	GP	in the presence of			NULL		NULL	NULL	NULL	NULL	gw60_science_280_5372_2109_s_59	9641915	( B) Hydrolysis of GTP bound to Galpha13 ( ) or Galpha12 ( ) was measured at 4 degrees C in the presence of the indicated concentrations of p115 RhoGEF.	bind
736	4	1152	7	10	NULL	0	NULL	statement 2	Process		undergoes hydrolysis					p115 RhoGEF	GP	in the presence of			NULL		NULL	NULL	NULL	NULL	gw60_science_280_5372_2109_s_59	9641915	( B) Hydrolysis of GTP bound to Galpha13 ( ) or Galpha12 ( ) was measured at 4 degrees C in the presence of the indicated concentrations of p115 RhoGEF.	bind
48846	2	1152	7	10	NULL	0	NULL	GTP	Chemical		bind					Galpha12	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_280_5372_2109_s_59	9641915	( B) Hydrolysis of GTP bound to Galpha13 ( ) or Galpha12 ( ) was measured at 4 degrees C in the presence of the indicated concentrations of p115 RhoGEF.	bind
942	1	1154	5	10	NULL	0	NULL	Stat1	GP		bind					DNA	NucleicAcid				NULL	WT MEFs	NULL	NULL	NULL	NULL	gw60_science_288_5475_2357_s_39	10875919	( B) IFN-gamma-induced  DNA-binding activities of Stat1 and ISGF3 in WT and  AR1 /  MEFs.	bind
943	2	1154	5	10	NULL	0	NULL	ISGF3	GP		bind					DNA	NucleicAcid				NULL	WT MEFs	NULL	NULL	NULL	NULL	gw60_science_288_5475_2357_s_39	10875919	( B) IFN-gamma-induced  DNA-binding activities of Stat1 and ISGF3 in WT and  AR1 /  MEFs.	bind
945	3	1154	5	10	NULL	0	NULL	IFN-gamma	GP		induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_288_5475_2357_s_39	10875919	( B) IFN-gamma-induced  DNA-binding activities of Stat1 and ISGF3 in WT and  AR1 /  MEFs.	bind
946	4	1154	5	10	NULL	0	NULL	IFN-gamma	GP		induce					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_288_5475_2357_s_39	10875919	( B) IFN-gamma-induced  DNA-binding activities of Stat1 and ISGF3 in WT and  AR1 /  MEFs.	bind
48847	5	1154	5	10	NULL	0	NULL	Stat1	GP		bind					DNA	NucleicAcid				NULL	AR1 MEFs	NULL	NULL	NULL	NULL	gw60_science_288_5475_2357_s_39	10875919	( B) IFN-gamma-induced  DNA-binding activities of Stat1 and ISGF3 in WT and  AR1 /  MEFs.	bind
48848	6	1154	5	10	NULL	0	NULL	ISGF3	GP		bind					DNA	NucleicAcid				NULL	AR1 MEFs	NULL	NULL	NULL	NULL	gw60_science_288_5475_2357_s_39	10875919	( B) IFN-gamma-induced  DNA-binding activities of Stat1 and ISGF3 in WT and  AR1 /  MEFs.	bind
48849	7	1154	5	10	NULL	0	NULL	IFN-gamma	GP		induces					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_288_5475_2357_s_39	10875919	( B) IFN-gamma-induced  DNA-binding activities of Stat1 and ISGF3 in WT and  AR1 /  MEFs.	bind
48850	8	1154	5	10	NULL	0	NULL	IFN-gamma	GP		induces					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_288_5475_2357_s_39	10875919	( B) IFN-gamma-induced  DNA-binding activities of Stat1 and ISGF3 in WT and  AR1 /  MEFs.	bind
747	1	1154	7	10	NULL	0	NULL	Stat1	GP		bind 					DNA	NucleicAcid				NULL	WT MEFs	NULL	NULL	NULL	NULL	gw60_science_288_5475_2357_s_39	10875919	( B) IFN-gamma-induced  DNA-binding activities of Stat1 and ISGF3 in WT and  AR1 /  MEFs.	bind
749	2	1154	7	10	NULL	0	NULL	Stat1	GP		bind					DNA	NucleicAcid				NULL	AR1 MEFs	NULL	NULL	NULL	NULL	gw60_science_288_5475_2357_s_39	10875919	( B) IFN-gamma-induced  DNA-binding activities of Stat1 and ISGF3 in WT and  AR1 /  MEFs.	bind
754	3	1154	7	10	NULL	0	NULL	ISGF3	GP		bind					DNA	NucleicAcid				NULL	WT MEFs	NULL	NULL	NULL	NULL	gw60_science_288_5475_2357_s_39	10875919	( B) IFN-gamma-induced  DNA-binding activities of Stat1 and ISGF3 in WT and  AR1 /  MEFs.	bind
755	4	1154	7	10	NULL	0	NULL	ISGF3	GP		bind					DNA	NucleicAcid				NULL	AR1 MEFs	NULL	NULL	NULL	NULL	gw60_science_288_5475_2357_s_39	10875919	( B) IFN-gamma-induced  DNA-binding activities of Stat1 and ISGF3 in WT and  AR1 /  MEFs.	bind
758	5	1154	7	10	NULL	0	NULL	IFN-gamma	GP		induces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_288_5475_2357_s_39	10875919	( B) IFN-gamma-induced  DNA-binding activities of Stat1 and ISGF3 in WT and  AR1 /  MEFs.	bind
760	6	1154	7	10	NULL	0	NULL	IFN-gamma	GP		induces					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_288_5475_2357_s_39	10875919	( B) IFN-gamma-induced  DNA-binding activities of Stat1 and ISGF3 in WT and  AR1 /  MEFs.	bind
761	8	1154	7	10	NULL	0	NULL	 IFN-gamma	GP		induces					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_288_5475_2357_s_39	10875919	( B) IFN-gamma-induced  DNA-binding activities of Stat1 and ISGF3 in WT and  AR1 /  MEFs.	bind
763	7	1154	7	10	NULL	0	NULL	 IFN-gamma	GP		induces					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_288_5475_2357_s_39	10875919	( B) IFN-gamma-induced  DNA-binding activities of Stat1 and ISGF3 in WT and  AR1 /  MEFs.	bind
947	1	1156	5	10	NULL	0	NULL	His6-Skn7p	GP	immobilized	bind					calcineurin	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_13_3473_s_167	11432834	( B) Immobilized His6-Skn7p binds calcineurin and Crz1p, but not GST.	bind
948	2	1156	5	10	NULL	0	NULL	His6-Skn7p	GP	immobilized	bind					Crz1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_13_3473_s_167	11432834	( B) Immobilized His6-Skn7p binds calcineurin and Crz1p, but not GST.	bind
769	1	1156	7	10	NULL	0	NULL	His6-Skn7p	GP	immobilized	bind					calcineurin	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_13_3473_s_167	11432834	( B) Immobilized His6-Skn7p binds calcineurin and Crz1p, but not GST.	bind
771	2	1156	7	10	NULL	0	NULL	His6-Skn7p	GP	immobilized 	bind					Crz1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_13_3473_s_167	11432834	( B) Immobilized His6-Skn7p binds calcineurin and Crz1p, but not GST.	bind
974	3	1158	5	NULL	NULL	0	NULL	mtHsp70	NULL		bind	NULL				Tim44	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevcelldevbiol_13_0_25_s_209	9442867	( b) Import motor (pulling); mtHsp70 bound to Tim44 interacts with the precursor polypeptide  ( Horst et al 1996).	bind
975	4	1158	5	NULL	NULL	0	NULL	mtHsp70	NULL	bound to Tim44	interact	NULL				precursor polypeptide	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevcelldevbiol_13_0_25_s_209	9442867	( b) Import motor (pulling); mtHsp70 bound to Tim44 interacts with the precursor polypeptide  ( Horst et al 1996).	bind
775	1	1158	7	NULL	NULL	0	NULL	mtHsp70	NULL		bind	NULL				 Tim44	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevcelldevbiol_13_0_25_s_209	9442867	( b) Import motor (pulling); mtHsp70 bound to Tim44 interacts with the precursor polypeptide  ( Horst et al 1996).	bind
776	5	1158	7	NULL	NULL	0	NULL	mtHsp70	NULL	Tim44 bound	interacts with	NULL				precursor polypeptide	NULL				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_13_0_25_s_209	9442867	( b) Import motor (pulling); mtHsp70 bound to Tim44 interacts with the precursor polypeptide  ( Horst et al 1996).	bind
979	1	1160	5	10	NULL	0	NULL	Scr/xd heterodimers	GP		bind									Hox/Exd-binding sites	NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_16_0_243_s_313	11031237	( B) In the activity regulation model, multiple Hox/Exd heterodimers (in this example,  Scr/xd and Antp/xd) bind to the same Hox/Exd-binding sites.	bind
980	2	1160	5	10	NULL	0	NULL	Antp/xd heterodimers	GP		bind									Hox/Exd-binding sites	NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_16_0_243_s_313	11031237	( B) In the activity regulation model, multiple Hox/Exd heterodimers (in this example,  Scr/xd and Antp/xd) bind to the same Hox/Exd-binding sites.	bind
778	1	1160	7	10	NULL	0	NULL	Scr/xd heterodimers	GP		bind									Hox/Exd-binding sites	NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_16_0_243_s_313	11031237	( B) In the activity regulation model, multiple Hox/Exd heterodimers (in this example,  Scr/xd and Antp/xd) bind to the same Hox/Exd-binding sites.	bind
779	2	1160	7	10	NULL	0	NULL	Antp/xd heterodimers 	GP		bind									Hox/Exd-binding sites	NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_16_0_243_s_313	11031237	( B) In the activity regulation model, multiple Hox/Exd heterodimers (in this example,  Scr/xd and Antp/xd) bind to the same Hox/Exd-binding sites.	bind
981	1	1162	5	10	NULL	0	NULL	p4	GP		bind					p6	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_22_6185_s_247	12426390	( B) In the presence of p6 and low concentrations of p4, a p4 - p6 complex is formed, but RNAP can still bind to the A2c promoter as a closed complex, although open complexes are not formed ( Camacho and Salas, 2001b).	bind
982	2	1162	5	10	NULL	0	NULL	RNAP	GP		bind					A2c	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_21_22_6185_s_247	12426390	( B) In the presence of p6 and low concentrations of p4, a p4 - p6 complex is formed, but RNAP can still bind to the A2c promoter as a closed complex, although open complexes are not formed ( Camacho and Salas, 2001b).	bind
47955	3	1162	5	10	NULL	0	NULL	statement 2	Process		occurs as a 					closed complex	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_22_6185_s_247	12426390	( B) In the presence of p6 and low concentrations of p4, a p4 - p6 complex is formed, but RNAP can still bind to the A2c promoter as a closed complex, although open complexes are not formed ( Camacho and Salas, 2001b).	bind
781	1	1162	7	10	NULL	0	NULL	p4	GP		bind					p6	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_22_6185_s_247	12426390	( B) In the presence of p6 and low concentrations of p4, a p4 - p6 complex is formed, but RNAP can still bind to the A2c promoter as a closed complex, although open complexes are not formed ( Camacho and Salas, 2001b).	bind
783	2	1162	7	10	NULL	0	NULL	RNAP	GP		bind					 A2c	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_21_22_6185_s_247	12426390	( B) In the presence of p6 and low concentrations of p4, a p4 - p6 complex is formed, but RNAP can still bind to the A2c promoter as a closed complex, although open complexes are not formed ( Camacho and Salas, 2001b).	bind
784	3	1162	7	10	NULL	0	NULL	statement 2	Process		occurs as a					closed complex	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_22_6185_s_247	12426390	( B) In the presence of p6 and low concentrations of p4, a p4 - p6 complex is formed, but RNAP can still bind to the A2c promoter as a closed complex, although open complexes are not formed ( Camacho and Salas, 2001b).	bind
983	1	1163	5	10	NULL	0	NULL	SacY	GP		bind					mRNA	NucleicAcid	nascent		RAT site	NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_22_12538_s_59	11606741	( B) In the presence of SacY, SacY binds to the RAT site in the nascent mRNA, causing antitermination so that transcription proceeds through the SacB'-'LacZ coding sequence and beta-galactosidase is formed.	bind
786	1	1163	7	10	NULL	0	NULL	SacY 	GP		bind 					mRNA	NucleicAcid	nascent		 RAT site	NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_22_12538_s_59	11606741	( B) In the presence of SacY, SacY binds to the RAT site in the nascent mRNA, causing antitermination so that transcription proceeds through the SacB'-'LacZ coding sequence and beta-galactosidase is formed.	bind
984	1	1164	5	10	NULL	0	NULL	HFR1	GP		bind					PIF3	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_genesdev_14_18_2377_s_197	10995393	( B) In vitro binding of HFR1 to PIF3.	bind
790	1	1164	7	10	NULL	0	NULL	HFR1	GP		bind					PIF3	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_genesdev_14_18_2377_s_197	10995393	( B) In vitro binding of HFR1 to PIF3.	bind
985	1	1165	5	10	NULL	0	NULL	CD11c+	GP	pulmonary APC	bind					pA:pU	Chemical	tagged			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jclininvest_110_8_1175_s_206	12393853	( b) In vivo binding of pulmonary CD11c+ and CD11b+ APCs by tagged pA:pU.	bind
986	2	1165	5	10	NULL	0	NULL	CD11b+	GP	pulmonary APC	bind					pA:pU	Chemical	tagged			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jclininvest_110_8_1175_s_206	12393853	( b) In vivo binding of pulmonary CD11c+ and CD11b+ APCs by tagged pA:pU.	bind
791	1	1165	7	10	NULL	0	NULL	CD11c+ 	GP	pulmonary APC	bind					pA:pU	Chemical	tagged			NULL	In vivo	NULL	NULL	NULL	NULL	gw60_jclininvest_110_8_1175_s_206	12393853	( b) In vivo binding of pulmonary CD11c+ and CD11b+ APCs by tagged pA:pU.	bind
792	2	1165	7	10	NULL	0	NULL	CD11b+ 	GP	pulmonary APC	bind					pA:pU	Chemical	tagged			NULL	In vivo	NULL	NULL	NULL	NULL	gw60_jclininvest_110_8_1175_s_206	12393853	( b) In vivo binding of pulmonary CD11c+ and CD11b+ APCs by tagged pA:pU.	bind
987	1	1170	5	10	NULL	0	NULL	Virus	Organism	radiolabelled	bind					BHK cells	Cell	live			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_3_543_s_53	9927414	( B) Inhibition of binding of radiolabelled virus to live BHK cells by heparin in the presence (dotted line) and absence (solid line) of a 100-fold excess of unlabelled virus.	bind
939	1	1170	7	10	NULL	0	NULL	Virus	Organism	radiolabelled 	bind					BHK cells	Cell	live			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_3_543_s_53	9927414	( B) Inhibition of binding of radiolabelled virus to live BHK cells by heparin in the presence (dotted line) and absence (solid line) of a 100-fold excess of unlabelled virus.	bind
992	1	1171	5	10	NULL	0	NULL	FasL	GP		bind					Fas receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_17_6599_s_93	15084739	( B) Inhibition of FasL binding to the Fas receptor by exocyclic peptidemimetics in a  binding assay.	bind
993	2	1171	5	10	NULL	0	NULL	peptidemimetics	Chemical	exocyclic	inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_17_6599_s_93	15084739	( B) Inhibition of FasL binding to the Fas receptor by exocyclic peptidemimetics in a  binding assay.	bind
944	1	1171	7	10	NULL	0	NULL	FasL	GP		bind					Fas receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_17_6599_s_93	15084739	( B) Inhibition of FasL binding to the Fas receptor by exocyclic peptidemimetics in a  binding assay.	bind
949	2	1171	7	10	NULL	0	NULL	peptidemimetics	Chemical	exocyclic 	inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_17_6599_s_93	15084739	( B) Inhibition of FasL binding to the Fas receptor by exocyclic peptidemimetics in a  binding assay.	bind
994	1	1172	5	10	NULL	0	NULL	importin-beta	GP		bind					NuMA	GP		tail II		NULL		NULL	NULL	NULL	NULL	gw60_science_291_5504_653_s_93	11229403	( B) Inhibition of importin-beta binding to NuMA tail II in extracts treated with RanL43E.	bind
995	2	1172	5	10	NULL	0	NULL	RanL43E	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_291_5504_653_s_93	11229403	( B) Inhibition of importin-beta binding to NuMA tail II in extracts treated with RanL43E.	bind
950	1	1172	7	10	NULL	0	NULL	importin-beta	GP		bind					NuMA 	GP		tail II		NULL		NULL	NULL	NULL	NULL	gw60_science_291_5504_653_s_93	11229403	( B) Inhibition of importin-beta binding to NuMA tail II in extracts treated with RanL43E.	bind
951	2	1172	7	10	NULL	0	NULL	RanL43E	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_291_5504_653_s_93	11229403	( B) Inhibition of importin-beta binding to NuMA tail II in extracts treated with RanL43E.	bind
996	1	1173	5	10	NULL	0	NULL	OspA peptide	GP	labeled	bind					TGE	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_106_4_561_s_98	10953031	( b) Inhibition of labeled OspA peptide binding to TGE by unlabeled OspA.	bind
997	2	1173	5	10	NULL	0	NULL	OspA	GP	unlabeled	inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_106_4_561_s_98	10953031	( b) Inhibition of labeled OspA peptide binding to TGE by unlabeled OspA.	bind
952	1	1173	7	10	NULL	0	NULL	OspA peptide	GP	labeled	bind					TGE	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_106_4_561_s_98	10953031	( b) Inhibition of labeled OspA peptide binding to TGE by unlabeled OspA.	bind
953	2	1173	7	10	NULL	0	NULL	OspA	GP	unlabeled	inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_106_4_561_s_98	10953031	( b) Inhibition of labeled OspA peptide binding to TGE by unlabeled OspA.	bind
998	1	1174	5	10	NULL	0	NULL	NF-kappaB	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_9_4844_s_183	10781090	( B) Inhibition of NF-kappaB DNA binding by cyclopentenone.	bind
999	2	1174	5	10	NULL	0	NULL	cyclopentenone	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_9_4844_s_183	10781090	( B) Inhibition of NF-kappaB DNA binding by cyclopentenone.	bind
954	1	1174	7	10	NULL	0	NULL	NF-kappaB	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_9_4844_s_183	10781090	( B) Inhibition of NF-kappaB DNA binding by cyclopentenone.	bind
955	2	1174	7	10	NULL	0	NULL	cyclopentenone	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_9_4844_s_183	10781090	( B) Inhibition of NF-kappaB DNA binding by cyclopentenone.	bind
1000	1	1175	5	10	NULL	0	NULL	biotin-HKa	GP		bind					tropomyosin	GP	purified			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_19_12224_s_157	12196635	( B) Inhibition of the binding of 20 nM biotin-HKa to purified tropomyosin by mAb TM-311.	bind
1001	2	1175	5	10	NULL	0	NULL	mAb TM-311	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_19_12224_s_157	12196635	( B) Inhibition of the binding of 20 nM biotin-HKa to purified tropomyosin by mAb TM-311.	bind
956	1	1175	7	10	NULL	0	NULL	biotin-HKa	GP		bind					tropomyosin	GP	purified			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_19_12224_s_157	12196635	( B) Inhibition of the binding of 20 nM biotin-HKa to purified tropomyosin by mAb TM-311.	bind
957	2	1175	7	10	NULL	0	NULL	mAb TM-311	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_19_12224_s_157	12196635	( B) Inhibition of the binding of 20 nM biotin-HKa to purified tropomyosin by mAb TM-311.	bind
1002	1	1176	5	10	NULL	0	NULL	A-p50	GP		bind					NF-kappaB p50 protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_12_3577_s_137	16855294	( B) Intracellular binding of A-p50 to NF-kappaB p50 protein.	bind
958	1	1176	7	10	NULL	0	NULL	 A-p50	GP		bind 					NF-kappaB p50 protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_12_3577_s_137	16855294	( B) Intracellular binding of A-p50 to NF-kappaB p50 protein.	bind
1005	1	1177	5	10	NULL	0	NULL	Ub	GP		bind								NZF		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1411_s_112	15029239	( B) Isotherms for Ub binding to wt and mutant NZF domains from Vps36p: wt Vps36-1 NZF  (black), Vps36-1 (T13G) NZF mutant (red), Vps36-1 (13TF14 to 13GS14) NZF mutant (blue), and wt Vps36-2 NZF (green).	bind
1006	2	1177	5	10	NULL	0	NULL	Ub	GP		bind								T13G;; NZF		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1411_s_112	15029239	( B) Isotherms for Ub binding to wt and mutant NZF domains from Vps36p: wt Vps36-1 NZF  (black), Vps36-1 (T13G) NZF mutant (red), Vps36-1 (13TF14 to 13GS14) NZF mutant (blue), and wt Vps36-2 NZF (green).	bind
1007	3	1177	5	10	NULL	0	NULL	Ub	GP		bind								13TF14 to 13GS14;; NZF		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1411_s_112	15029239	( B) Isotherms for Ub binding to wt and mutant NZF domains from Vps36p: wt Vps36-1 NZF  (black), Vps36-1 (T13G) NZF mutant (red), Vps36-1 (13TF14 to 13GS14) NZF mutant (blue), and wt Vps36-2 NZF (green).	bind
1008	4	1177	5	10	NULL	0	NULL	Ub	GP		bind								NZF		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1411_s_112	15029239	( B) Isotherms for Ub binding to wt and mutant NZF domains from Vps36p: wt Vps36-1 NZF  (black), Vps36-1 (T13G) NZF mutant (red), Vps36-1 (13TF14 to 13GS14) NZF mutant (blue), and wt Vps36-2 NZF (green).	bind
61093	5	1177	5	10	NULL	0	NULL	statement 1	Process		derived from			NZF		Vps36-1	GP	wt			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1411_s_112	15029239	( B) Isotherms for Ub binding to wt and mutant NZF domains from Vps36p: wt Vps36-1 NZF  (black), Vps36-1 (T13G) NZF mutant (red), Vps36-1 (13TF14 to 13GS14) NZF mutant (blue), and wt Vps36-2 NZF (green).	bind
61094	6	1177	5	10	NULL	0	NULL	statement 2	Process		derived from			NZF		Vps36-1	GP	mutant	T13G		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1411_s_112	15029239	( B) Isotherms for Ub binding to wt and mutant NZF domains from Vps36p: wt Vps36-1 NZF  (black), Vps36-1 (T13G) NZF mutant (red), Vps36-1 (13TF14 to 13GS14) NZF mutant (blue), and wt Vps36-2 NZF (green).	bind
61095	7	1177	5	10	NULL	0	NULL	statement 3	Process		derived from			NZF		Vps36-1	GP	mutant	13TF14 to 13GS14		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1411_s_112	15029239	( B) Isotherms for Ub binding to wt and mutant NZF domains from Vps36p: wt Vps36-1 NZF  (black), Vps36-1 (T13G) NZF mutant (red), Vps36-1 (13TF14 to 13GS14) NZF mutant (blue), and wt Vps36-2 NZF (green).	bind
61096	8	1177	5	10	NULL	0	NULL	statement 4	Process		derived from			NZF		Vps36-2	GP	wt			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1411_s_112	15029239	( B) Isotherms for Ub binding to wt and mutant NZF domains from Vps36p: wt Vps36-1 NZF  (black), Vps36-1 (T13G) NZF mutant (red), Vps36-1 (13TF14 to 13GS14) NZF mutant (blue), and wt Vps36-2 NZF (green).	bind
959	3	1177	7	10	NULL	0	NULL	Ub	GP		bind								NZF		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1411_s_112	15029239	( B) Isotherms for Ub binding to wt and mutant NZF domains from Vps36p: wt Vps36-1 NZF  (black), Vps36-1 (T13G) NZF mutant (red), Vps36-1 (13TF14 to 13GS14) NZF mutant (blue), and wt Vps36-2 NZF (green).	bind
960	1	1177	7	10	NULL	0	NULL	Ub	GP		bind								T13G;;NZF 		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1411_s_112	15029239	( B) Isotherms for Ub binding to wt and mutant NZF domains from Vps36p: wt Vps36-1 NZF  (black), Vps36-1 (T13G) NZF mutant (red), Vps36-1 (13TF14 to 13GS14) NZF mutant (blue), and wt Vps36-2 NZF (green).	bind
961	2	1177	7	10	NULL	0	NULL	Ub	GP		bind								13TF14 to 13GS14;;NZF		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1411_s_112	15029239	( B) Isotherms for Ub binding to wt and mutant NZF domains from Vps36p: wt Vps36-1 NZF  (black), Vps36-1 (T13G) NZF mutant (red), Vps36-1 (13TF14 to 13GS14) NZF mutant (blue), and wt Vps36-2 NZF (green).	bind
962	4	1177	7	10	NULL	0	NULL	Ub	GP		bind 								 NZF		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1411_s_112	15029239	( B) Isotherms for Ub binding to wt and mutant NZF domains from Vps36p: wt Vps36-1 NZF  (black), Vps36-1 (T13G) NZF mutant (red), Vps36-1 (13TF14 to 13GS14) NZF mutant (blue), and wt Vps36-2 NZF (green).	bind
61097	5	1177	7	10	NULL	0	NULL	statement 1	Process		derived from			NZF		Vps36-1	GP	wt			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1411_s_112	15029239	( B) Isotherms for Ub binding to wt and mutant NZF domains from Vps36p: wt Vps36-1 NZF  (black), Vps36-1 (T13G) NZF mutant (red), Vps36-1 (13TF14 to 13GS14) NZF mutant (blue), and wt Vps36-2 NZF (green).	bind
61098	6	1177	7	10	NULL	0	NULL	statement 2	Process		derived from			NZF		Vps36-1	GP	mutant	T13G		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1411_s_112	15029239	( B) Isotherms for Ub binding to wt and mutant NZF domains from Vps36p: wt Vps36-1 NZF  (black), Vps36-1 (T13G) NZF mutant (red), Vps36-1 (13TF14 to 13GS14) NZF mutant (blue), and wt Vps36-2 NZF (green).	bind
61099	7	1177	7	10	NULL	0	NULL	statement 3	Process		derived from			NZF		Vps36-1	GP	mutant	13TF14 to 13GS14		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1411_s_112	15029239	( B) Isotherms for Ub binding to wt and mutant NZF domains from Vps36p: wt Vps36-1 NZF  (black), Vps36-1 (T13G) NZF mutant (red), Vps36-1 (13TF14 to 13GS14) NZF mutant (blue), and wt Vps36-2 NZF (green).	bind
61100	8	1177	7	10	NULL	0	NULL	statement 4	Process		derived from			NZF		Vps36-2	GP	wt			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1411_s_112	15029239	( B) Isotherms for Ub binding to wt and mutant NZF domains from Vps36p: wt Vps36-1 NZF  (black), Vps36-1 (T13G) NZF mutant (red), Vps36-1 (13TF14 to 13GS14) NZF mutant (blue), and wt Vps36-2 NZF (green).	bind
1009	1	1178	5	10	NULL	0	NULL	ISWI	GP		bind					H2A nucleosomes	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_19_3815_s_98	15372075	( B) ISWI binding to the H2A and H2ABbd nucleosomes.	bind
1010	2	1178	5	10	NULL	0	NULL	ISWI	GP		bind					H2ABbd nucleosomes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_19_3815_s_98	15372075	( B) ISWI binding to the H2A and H2ABbd nucleosomes.	bind
963	1	1178	7	10	NULL	0	NULL	 ISWI	GP		bind					H2A nucleosomes	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_19_3815_s_98	15372075	( B) ISWI binding to the H2A and H2ABbd nucleosomes.	bind
964	2	1178	7	10	NULL	0	NULL	ISWI	GP		bind					H2ABbd nucleosomes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_19_3815_s_98	15372075	( B) ISWI binding to the H2A and H2ABbd nucleosomes.	bind
1014	1	1179	5	10	NULL	0	NULL	CypA	GP		bind					Itk	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_4_1899_s_156	11830645	( b) Itk phosphorylation following TCR stimulation of Jurkat cells in the presence and absence of CsA. ( c) CypA binding to Itk was monitored by detection of Itk immunoprecipitates with an anti-CypA antibody.	bind
1015	2	1179	5	10	NULL	0	NULL	TCR	GP		stimulate					Itk	GP	phosphorylation of			NULL	Jurkat cells	NULL	NULL	NULL	NULL	gw60_pnas_99_4_1899_s_156	11830645	( b) Itk phosphorylation following TCR stimulation of Jurkat cells in the presence and absence of CsA. ( c) CypA binding to Itk was monitored by detection of Itk immunoprecipitates with an anti-CypA antibody.	bind
965	1	1179	7	10	NULL	0	NULL	TCR	GP		stimulate					Itk	GP	phosphorylation of			NULL	Jurkat cells	NULL	NULL	NULL	NULL	gw60_pnas_99_4_1899_s_156	11830645	( b) Itk phosphorylation following TCR stimulation of Jurkat cells in the presence and absence of CsA. ( c) CypA binding to Itk was monitored by detection of Itk immunoprecipitates with an anti-CypA antibody.	bind
969	2	1179	7	10	NULL	0	NULL	CypA	GP		bind					Itk	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_4_1899_s_156	11830645	( b) Itk phosphorylation following TCR stimulation of Jurkat cells in the presence and absence of CsA. ( c) CypA binding to Itk was monitored by detection of Itk immunoprecipitates with an anti-CypA antibody.	bind
1016	1	1180	5	10	NULL	0	NULL	JNK	GP		bind					p53	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_17_2658_s_30	9732264	( b) JNK binding to p53 is inhibited by p7.	bind
1017	2	1180	5	10	NULL	0	NULL	p7	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_17_2658_s_30	9732264	( b) JNK binding to p53 is inhibited by p7.	bind
970	1	1180	7	10	NULL	0	NULL	JNK	GP		bind					 p53	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_17_2658_s_30	9732264	( b) JNK binding to p53 is inhibited by p7.	bind
971	2	1180	7	10	NULL	0	NULL	p7	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_17_2658_s_30	9732264	( b) JNK binding to p53 is inhibited by p7.	bind
1051	1	1181	5	10	NULL	0	NULL	spt	GP		does not bind			K145E ( spt15-640)		TFIIA	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_23_6662_s_162	10581240	( B) K145E ( spt15-640) fails to bind TFIIA.	bind
976	1	1181	7	10	NULL	0	NULL	spt	GP		does not bind			K145E ( spt15-640)		TFIIA	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_23_6662_s_162	10581240	( B) K145E ( spt15-640) fails to bind TFIIA.	bind
1052	1	1182	5	10	NULL	0	NULL	kappaB-DNA	GP		bind		preferentially			p50 homodimer	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_16_9268_s_26	12886018	( b) kappaB-DNA  sequences that preferentially bind the p50 homodimer ( Upper) and  p50/p65 heterodimer ( Lower) are shown.	bind
1053	2	1182	5	10	NULL	0	NULL	kappaB-DNA	GP		bind		preferentially			p50/p65 heterodimer	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_16_9268_s_26	12886018	( b) kappaB-DNA  sequences that preferentially bind the p50 homodimer ( Upper) and  p50/p65 heterodimer ( Lower) are shown.	bind
977	1	1182	7	10	NULL	0	NULL	kappaB-DNA	GP		bind		preferentially			p50 homodimer	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_16_9268_s_26	12886018	( b) kappaB-DNA  sequences that preferentially bind the p50 homodimer ( Upper) and  p50/p65 heterodimer ( Lower) are shown.	bind
978	2	1182	7	10	NULL	0	NULL	kappaB-DNA	GP		bind		preferentially 			p50/p65 heterodimer	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_16_9268_s_26	12886018	( b) kappaB-DNA  sequences that preferentially bind the p50 homodimer ( Upper) and  p50/p65 heterodimer ( Lower) are shown.	bind
1054	1	1183	5	10	NULL	0	NULL	gp120	GP	core	bind					CD4 surface	Cell				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_16_9026_s_148	10922058	( B) Kinetic data set collected for core gp120 binding to a CD4 surface.	bind
1018	1	1183	7	10	NULL	0	NULL	gp120	GP	core	bind					CD4 surface	Cell				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_16_9026_s_148	10922058	( B) Kinetic data set collected for core gp120 binding to a CD4 surface.	bind
1055	1	1185	5	10	NULL	0	NULL	FGF-2	GP		associate					Namalwa	Cell	transfectants			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_111_8_1211_s_152	12697740	( b) Kinetics of FGFR-1 binding to FGF-2 - associated Namalwa transfectants.	bind
1056	2	1185	5	10	NULL	0	NULL	FGFR-1	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_111_8_1211_s_152	12697740	( b) Kinetics of FGFR-1 binding to FGF-2 - associated Namalwa transfectants.	bind
1021	1	1185	7	10	NULL	0	NULL	FGF2	GP		associate					Namalwa	Cell	transfectants			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_111_8_1211_s_152	12697740	( b) Kinetics of FGFR-1 binding to FGF-2 - associated Namalwa transfectants.	bind
1262	2	1185	7	10	NULL	0	NULL	FGFR-1	GP		bind 					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_111_8_1211_s_152	12697740	( b) Kinetics of FGFR-1 binding to FGF-2 - associated Namalwa transfectants.	bind
47956	1	1186	5	10	NULL	0	NULL	PNA I	GP		bind					pSD1	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_9_5953_s_59	11972051	( b) Kinetics of PNA I binding to pSD1 target as monitored by gel-shift assay.	bind
1022	1	1186	7	10	NULL	0	NULL	PNA I	GP		bind					pSD1	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_9_5953_s_59	11972051	( b) Kinetics of PNA I binding to pSD1 target as monitored by gel-shift assay.	bind
1057	1	1187	5	10	NULL	0	NULL	GST-PDZ2	GP		bind					CFTR	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_3_1300_s_138	11158634	( B) Kinetics-response data for GST-PDZ2 binding to CFTR.	bind
1023	1	1187	7	10	NULL	0	NULL	GST-PDZ2	GP		bind					CFTR	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_3_1300_s_138	11158634	( B) Kinetics-response data for GST-PDZ2 binding to CFTR.	bind
1058	1	1188	5	10	NULL	0	NULL	Ku	GP		bind					IP6	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_19_5501_s_176	14500812	( b) Ku binding to IP6.	bind
1024	1	1188	7	10	NULL	0	NULL	Ku	GP		bind					IP6	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_19_5501_s_176	14500812	( b) Ku binding to IP6.	bind
1059	1	1189	5	10	NULL	0	NULL	L525P-Axin 	GP		does not bind					GSK-3beta	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_9_1066_s_100	12000790	( b) L525P-Axin does not bind GSK-3beta.	bind
1025	1	1189	7	10	NULL	0	NULL	L525P-Axin	GP		does not bind					GSK-3beta	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_9_1066_s_100	12000790	( b) L525P-Axin does not bind GSK-3beta.	bind
1060	1	1190	5	10	NULL	0	NULL	LARG	GP		bind		directly	PDZ		plexin-B1	GP		C terminus		NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_19_12085_s_192	12196628	( B) LARG-PDZ directly binds the C terminus of plexin-B1.	bind
1026	1	1190	7	10	NULL	0	NULL	LARG	GP		bind 		directly	PDZ		plexin-B1	GP		C terminus		NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_19_12085_s_192	12196628	( B) LARG-PDZ directly binds the C terminus of plexin-B1.	bind
1061	1	1191	5	10	NULL	0	NULL	Lectin	GP		bind					Reelin	GP				NULL	CSF samples	NULL	NULL	NULL	NULL	gw70_pnas_103_14_5573_s_114	16567613	( B) Lectin binding of 180-kDa Reelin in gender- and age-matched CSF samples for 9 NDC  and 11 AD subjects.	bind
1027	1	1191	7	10	NULL	0	NULL	Lectin	GP		bind					Reelin	GP				NULL	CSF samples	NULL	NULL	NULL	NULL	gw70_pnas_103_14_5573_s_114	16567613	( B) Lectin binding of 180-kDa Reelin in gender- and age-matched CSF samples for 9 NDC  and 11 AD subjects.	bind
1062	1	1193	5	10	NULL	0	NULL	PI(3,4,5)P3	Chemical		bind					GST-PLCgamma1	GP		PH		NULL		NULL	NULL	NULL	NULL	gw60_embo_17_2_414_s_52	9430633	( B) Ligand displacement of [32]gPI(3,4,5)P3 binding to GST-PLCgamma1-PH by Ins(1,3,4,5)P4.	bind
1063	2	1193	5	10	NULL	0	NULL	Ins(1,3,4,5)P4	Chemical		bind					GST-PLCgamma1	GP		PH		NULL		NULL	NULL	NULL	NULL	gw60_embo_17_2_414_s_52	9430633	( B) Ligand displacement of [32]gPI(3,4,5)P3 binding to GST-PLCgamma1-PH by Ins(1,3,4,5)P4.	bind
1028	1	1193	7	10	NULL	0	NULL	PI(3,4,5)P3	Chemical		bind					GST-PLCgamma1	GP		PH		NULL		NULL	NULL	NULL	NULL	gw60_embo_17_2_414_s_52	9430633	( B) Ligand displacement of [32]gPI(3,4,5)P3 binding to GST-PLCgamma1-PH by Ins(1,3,4,5)P4.	bind
1029	2	1193	7	10	NULL	0	NULL	Ins(1,3,4,5)P4	Chemical		bind					GST-PLCgamma1	GP		PH		NULL		NULL	NULL	NULL	NULL	gw60_embo_17_2_414_s_52	9430633	( B) Ligand displacement of [32]gPI(3,4,5)P3 binding to GST-PLCgamma1-PH by Ins(1,3,4,5)P4.	bind
1064	1	1194	5	10	NULL	0	NULL	LC13 TcR	GP		bind					FLR - HLA-B8 complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_17_6641_s_99	16617112	( B) Ligated conformation of the LC13 TcR bound to the FLR - HLA-B8 complex (purple).	bind
1030	1	1194	7	10	NULL	0	NULL	LC13 TcR	GP		bind					FLR - HLA-B8 complex 	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_17_6641_s_99	16617112	( B) Ligated conformation of the LC13 TcR bound to the FLR - HLA-B8 complex (purple).	bind
1066	1	1197	5	10	NULL	0	NULL	LSm protein	GP		bind					U6	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_20_5789_s_255	10523320	( B) LSm protein binding of the U6 mutants.	bind
1032	1	1197	7	10	NULL	0	NULL	LSm protein	GP		bind					U6 	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_20_5789_s_255	10523320	( B) LSm protein binding of the U6 mutants.	bind
1067	1	1198	5	10	NULL	0	NULL	cell wall	Cell	maize	bind					EXPB1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_40_14664_s_140	16984999	( B) Maize cell walls bind EXPB1.	bind
1033	1	1198	7	10	NULL	0	NULL	cell wall	Cell	Maize 	bind 					EXPB1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_40_14664_s_140	16984999	( B) Maize cell walls bind EXPB1.	bind
1068	1	1199	5	10	NULL	0	NULL	VEGF	GP		bind					VEGFR2	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_22_12485_s_211	11606713	( B) Mammary tumor sections from TgN-neu (a-c), neu-hTSP1 (d-f), neu- tbsp1  /  (g-i) mice were evaluated for expression of VEGF by using two antibodies: GV39 M, which recognizes VEGF bound to VEGFR2 (b, e, h) and a polyclonal anti-mouse VEGF, which recognizes the receptor-free form (c, f, i).	bind
1034	1	1199	7	10	NULL	0	NULL	VEGF 	GP		bind					VEGFR2	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_22_12485_s_211	11606713	( B) Mammary tumor sections from TgN-neu (a-c), neu-hTSP1 (d-f), neu- tbsp1  /  (g-i) mice were evaluated for expression of VEGF by using two antibodies: GV39 M, which recognizes VEGF bound to VEGFR2 (b, e, h) and a polyclonal anti-mouse VEGF, which recognizes the receptor-free form (c, f, i).	bind
1087	1	1231	6	NULL	NULL	0	NULL	p21	NULL		bind	NULL				PCNA	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_4_1392_s_124	9465025	( B) p21 and p57 bind to PCNA via similar sequences.	bind
1088	2	1231	6	NULL	NULL	0	NULL	p57	NULL		bind	NULL				PCNA	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_4_1392_s_124	9465025	( B) p21 and p57 bind to PCNA via similar sequences.	bind
1092	1	1245	6	NULL	NULL	0	NULL	PGC-1	NULL		bind	NULL				SRC-1	NULL				NULL	cells	NULL	NULL	NULL	NULL	gw60_science_286_5443_1368_s_109	10558993	( B) PPARgamma and NRF-1 increase the binding of PGC-1 to SRC-1 and p300 in cells.	bind
1093	2	1245	6	NULL	NULL	0	NULL	PGC-1	NULL		bind	NULL				p300	NULL				NULL	cells	NULL	NULL	NULL	NULL	gw60_science_286_5443_1368_s_109	10558993	( B) PPARgamma and NRF-1 increase the binding of PGC-1 to SRC-1 and p300 in cells.	bind
1094	3	1245	6	NULL	NULL	0	NULL	PPARgamma	NULL		increases	NULL				Statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_science_286_5443_1368_s_109	10558993	( B) PPARgamma and NRF-1 increase the binding of PGC-1 to SRC-1 and p300 in cells.	bind
1095	4	1245	6	NULL	NULL	0	NULL	PPARgamma	NULL		increases	NULL				Statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_science_286_5443_1368_s_109	10558993	( B) PPARgamma and NRF-1 increase the binding of PGC-1 to SRC-1 and p300 in cells.	bind
1096	5	1245	6	NULL	NULL	0	NULL	NRF-1	NULL		increases	NULL				Statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_science_286_5443_1368_s_109	10558993	( B) PPARgamma and NRF-1 increase the binding of PGC-1 to SRC-1 and p300 in cells.	bind
1097	6	1245	6	NULL	NULL	0	NULL	NRF-1	NULL		increases	NULL				Statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_science_286_5443_1368_s_109	10558993	( B) PPARgamma and NRF-1 increase the binding of PGC-1 to SRC-1 and p300 in cells.	bind
1142	5	1401	5	NULL	NULL	0	NULL	Yan monomer	NULL	phosphorylation	favor	NULL				Crm1	NULL	binding			NULL		0	NULL	NULL	NULL	gw70_genesdev_19_15_1767_s_120	16027171	( B) Upon RTK activation, phosphorylation of the Yan monomer favors Crm1 binding, leading  to the export of the Yan monomer.	bind
1143	6	1401	5	NULL	NULL	0	NULL	RTK	NULL	activation	required for	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_15_1767_s_120	16027171	( B) Upon RTK activation, phosphorylation of the Yan monomer favors Crm1 binding, leading  to the export of the Yan monomer.	bind
1144	7	1401	5	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				Yan monomer	NULL	export			NULL		0	NULL	NULL	NULL	gw70_genesdev_19_15_1767_s_120	16027171	( B) Upon RTK activation, phosphorylation of the Yan monomer favors Crm1 binding, leading  to the export of the Yan monomer.	bind
1035	12	1401	7	NULL	NULL	0	NULL	Yan monomer	NULL	 phosphorylated 	bind	NULL				Crm1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_15_1767_s_120	16027171	( B) Upon RTK activation, phosphorylation of the Yan monomer favors Crm1 binding, leading  to the export of the Yan monomer.	bind
1038	13	1401	7	NULL	NULL	0	NULL	statement 12	NULL		leads to 	NULL				Yan monomer	NULL	the export of 			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_15_1767_s_120	16027171	( B) Upon RTK activation, phosphorylation of the Yan monomer favors Crm1 binding, leading  to the export of the Yan monomer.	bind
1583	14	1401	7	NULL	NULL	0	NULL	RTK	NULL	activation of 	required for	NULL				statement 12	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_15_1767_s_120	16027171	( B) Upon RTK activation, phosphorylation of the Yan monomer favors Crm1 binding, leading  to the export of the Yan monomer.	bind
1145	1	1402	5	10	NULL	0	NULL	ATP	Chemical		bind					Hsp104	GP		Y819W		NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_5_2732_s_190	11867765	( B) Urea denaturation of  Hsp104549-908 R826M monitored by CD at 225 nm. ATP ( C) and ADP ( D) binding to Hsp104Y819W R826M fit to a single-site Hill equation.	bind
1146	2	1402	5	10	NULL	0	NULL	ADP	Chemical		bind					Hsp104	GP		Y819W		NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_5_2732_s_190	11867765	( B) Urea denaturation of  Hsp104549-908 R826M monitored by CD at 225 nm. ATP ( C) and ADP ( D) binding to Hsp104Y819W R826M fit to a single-site Hill equation.	bind
1197	1	1402	7	10	NULL	0	NULL	ATP	Chemical		bind					Hsp104	GP		Y819W		NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_5_2732_s_190	11867765	( B) Urea denaturation of  Hsp104549-908 R826M monitored by CD at 225 nm. ATP ( C) and ADP ( D) binding to Hsp104Y819W R826M fit to a single-site Hill equation.	bind
1198	2	1402	7	10	NULL	0	NULL	ADP	Chemical		bind					Hsp104	GP		Y819W		NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_5_2732_s_190	11867765	( B) Urea denaturation of  Hsp104549-908 R826M monitored by CD at 225 nm. ATP ( C) and ADP ( D) binding to Hsp104Y819W R826M fit to a single-site Hill equation.	bind
1147	1	1403	5	10	NULL	0	NULL	ATP	Chemical		bind					TAP1	GP	single chain			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_387_s_155	11157746	( B) US6 does not inhibit ATP binding by single chain TAP1.	bind
1148	2	1403	5	10	NULL	0	NULL	US6	GP		does not inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_387_s_155	11157746	( B) US6 does not inhibit ATP binding by single chain TAP1.	bind
1199	1	1403	7	10	NULL	0	NULL	ATP	Chemical		bind					TAP1	GP	single chain			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_387_s_155	11157746	( B) US6 does not inhibit ATP binding by single chain TAP1.	bind
1200	2	1403	7	10	NULL	0	NULL	US6	GP		does not inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_387_s_155	11157746	( B) US6 does not inhibit ATP binding by single chain TAP1.	bind
1149	1	1404	5	NULL	NULL	0	NULL	USF-1	NULL		bind	NULL				lama3	NULL			promoter	NULL	in vivo	0	NULL	NULL	NULL	gw60_nucleicacidsres_30_8_1789_s_134	11937633	( B) USF-1 binds the  lama3 promoter  in vivo.	bind
1201	3	1404	7	NULL	NULL	0	NULL	USF-1	NULL		bind	NULL				lama3 	NULL			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_8_1789_s_134	11937633	( B) USF-1 binds the  lama3 promoter  in vivo.	bind
1151	1	1406	5	10	NULL	0	NULL	VDR-RXR heterodimers	GP		bind					CYP3A 	GP			VDRE	NULL		NULL	NULL	NULL	NULL	gw60_science_296_5571_1313_s_90	12016314	( B) VDR-RXR heterodimers bind to CYP3A VDREs.	bind
1202	2	1406	7	10	NULL	0	NULL	VDR-RXR heterodimers	GP		bind					CYP3A 	GP			VDRE	NULL		NULL	NULL	NULL	NULL	gw60_science_296_5571_1313_s_90	12016314	( B) VDR-RXR heterodimers bind to CYP3A VDREs.	bind
1152	1	1407	5	10	NULL	0	NULL	Vinculin	GP		bind					IpaA	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_5853_s_77	10545097	( B) Vinculin binding to IpaA is inhibited by MBPV1-265.	bind
1153	2	1407	5	10	NULL	0	NULL	MBPV1-265	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_5853_s_77	10545097	( B) Vinculin binding to IpaA is inhibited by MBPV1-265.	bind
1203	1	1407	7	10	NULL	0	NULL	Vinculin	GP		bind					IpaA	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_5853_s_77	10545097	( B) Vinculin binding to IpaA is inhibited by MBPV1-265.	bind
1204	2	1407	7	10	NULL	0	NULL	MBPV1-265	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_5853_s_77	10545097	( B) Vinculin binding to IpaA is inhibited by MBPV1-265.	bind
1154	1	1409	5	10	NULL	0	NULL	reelin	GP		bind					SNSs	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_9_5479_s_164	12707415	( B) Western immunoblot of reelin bound to SNSs after incubation with or without reelin in the presence or absence of different doses of rapamycin.	bind
1205	1	1409	7	10	NULL	0	NULL	reelin	GP		bind to					SNSs	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_9_5479_s_164	12707415	( B) Western immunoblot of reelin bound to SNSs after incubation with or without reelin in the presence or absence of different doses of rapamycin.	bind
1155	1	1410	5	10	NULL	0	NULL	Hh	GP		bind					Ptc	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_13_3505_s_42	9649421	( B) When Hh binds to Ptc, the inhibitory effect on Smo is suppressed.	bind
1156	2	1410	5	10	NULL	0	NULL	statement 1	Process		suppresses					Smo	GP	inhibitory effect on			NULL		NULL	NULL	NULL	NULL	gw60_embo_17_13_3505_s_42	9649421	( B) When Hh binds to Ptc, the inhibitory effect on Smo is suppressed.	bind
1281	1	1410	7	10	NULL	0	NULL	Hh	GP		bind 					 Ptc	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_13_3505_s_42	9649421	( B) When Hh binds to Ptc, the inhibitory effect on Smo is suppressed.	bind
1284	2	1410	7	10	NULL	0	NULL	statement 1	Process		suppresses					Smo	GP	inhibitory effect on 			NULL		NULL	NULL	NULL	NULL	gw60_embo_17_13_3505_s_42	9649421	( B) When Hh binds to Ptc, the inhibitory effect on Smo is suppressed.	bind
1157	1	1411	5	10	NULL	0	NULL	MTs	CellComponent		bind					kinetochore	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_18_0_193_s_328	12142285	( B) When MTs bind a kinetochore, they prevent future CP activation either by competing  for kinetochore-binding sites or by some mechanism for active removal ( straight arrows), perhaps by removing them from the kinetochore with minus end-directed motors.	bind
1158	2	1411	5	10	NULL	0	NULL	statement 1	Process		prevent					CP	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_18_0_193_s_328	12142285	( B) When MTs bind a kinetochore, they prevent future CP activation either by competing  for kinetochore-binding sites or by some mechanism for active removal ( straight arrows), perhaps by removing them from the kinetochore with minus end-directed motors.	bind
1287	1	1411	7	10	NULL	0	NULL	MTs	CellComponent		bind 					kinetochore	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_18_0_193_s_328	12142285	( B) When MTs bind a kinetochore, they prevent future CP activation either by competing  for kinetochore-binding sites or by some mechanism for active removal ( straight arrows), perhaps by removing them from the kinetochore with minus end-directed motors.	bind
1288	2	1411	7	10	NULL	0	NULL	statement 1	Process		prevent					CP	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_18_0_193_s_328	12142285	( B) When MTs bind a kinetochore, they prevent future CP activation either by competing  for kinetochore-binding sites or by some mechanism for active removal ( straight arrows), perhaps by removing them from the kinetochore with minus end-directed motors.	bind
1159	1	1412	5	10	NULL	0	NULL	TBP	GP		bind					BNA1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_174	15861138	( B) Wild-type ( TAF1) and  taf1 cells were grown and heat-shocked as in panel A. TBP binding to the  BNA1 and  URA1 promoters was then determined by ChIP.	bind
1160	2	1412	5	10	NULL	0	NULL	TBP	GP		bind					 URA1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_174	15861138	( B) Wild-type ( TAF1) and  taf1 cells were grown and heat-shocked as in panel A. TBP binding to the  BNA1 and  URA1 promoters was then determined by ChIP.	bind
1388	3	1412	7	10	NULL	0	NULL	TBP	GP		bind					BNA1	GP			 promoter	NULL		NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_174	15861138	( B) Wild-type ( TAF1) and  taf1 cells were grown and heat-shocked as in panel A. TBP binding to the  BNA1 and  URA1 promoters was then determined by ChIP.	bind
1389	4	1412	7	10	NULL	0	NULL	TBP	GP		bind					URA1 	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_174	15861138	( B) Wild-type ( TAF1) and  taf1 cells were grown and heat-shocked as in panel A. TBP binding to the  BNA1 and  URA1 promoters was then determined by ChIP.	bind
1161	1	1413	5	10	NULL	0	NULL	WT1	GP		bind					GST-U2AF65	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_20_3217_s_84	9784496	( B) WT1 binding to GST-U2AF65 compared to GST alone under different salt concentrations.	bind
1398	1	1413	7	10	NULL	0	NULL	WT1	GP		bind					GST-U2AF65	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_20_3217_s_84	9784496	( B) WT1 binding to GST-U2AF65 compared to GST alone under different salt concentrations.	bind
1162	1	1414	5	10	NULL	0	NULL	dCLOCK-dBMAL1 heterodimer	GP		bind					per	GP			E-box site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_science_280_5369_1599_s_146	9616122	( B) Yeast one-hybrid assay showing binding of the dCLOCK-dBMAL1 heterodimer to the  per E-box site.	bind
1399	1	1414	7	10	NULL	0	NULL	dCLOCK-dBMAL1 heterodimer	GP		bind					per	GP			E-box site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_science_280_5369_1599_s_146	9616122	( B) Yeast one-hybrid assay showing binding of the dCLOCK-dBMAL1 heterodimer to the  per E-box site.	bind
1163	1	1415	5	NULL	NULL	0	NULL	GRIP	NULL		bind	NULL	selectively	PDZ domain 6		SR	NULL				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_6_2105_s_116	15684087	( B) Yeast two-hybrid analysis establishes selective binding of GRIP's PDZ domain  6 to SR. ( C and  D) Yeast two-hybrid analysis was used to determine which region of SR interacts with  GRIP.	bind
1401	3	1415	7	NULL	NULL	0	NULL	GRIP	NULL		bind to	NULL	selectively	PDZ domain 6		SR	NULL				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_6_2105_s_116	15684087	( B) Yeast two-hybrid analysis establishes selective binding of GRIP's PDZ domain  6 to SR. ( C and  D) Yeast two-hybrid analysis was used to determine which region of SR interacts with  GRIP.	bind
1164	1	1416	5	10	NULL	0	NULL	YopJ	GP		bind		specifically			GST-MKK1	GP	recombinant			NULL		NULL	NULL	NULL	NULL	gw60_science_285_5435_1920_s_35	10489373	( B) YopJ specifically bound recombinant GST-MKK1, GST-MKK3, GST-MKK4/SEK1, and GST-MKK5 but not GST. 35S-methionine-labeled pcDNA3-YopJ was incubated with bacterially expressed recombinant GST (lane 2), GST-MKK1 (lane 3), GST-MKK3 (lane 4), GST-MKK4/SEK1 (lane 5), or GST-MKK5 (lane 6) bound to glutathione-agarose and analyzed as previously described ( 29,  30).	bind
1165	2	1416	5	10	NULL	0	NULL	YopJ	GP		bind		specifically			GST-MKK3	GP	recombinant			NULL		NULL	NULL	NULL	NULL	gw60_science_285_5435_1920_s_35	10489373	( B) YopJ specifically bound recombinant GST-MKK1, GST-MKK3, GST-MKK4/SEK1, and GST-MKK5 but not GST. 35S-methionine-labeled pcDNA3-YopJ was incubated with bacterially expressed recombinant GST (lane 2), GST-MKK1 (lane 3), GST-MKK3 (lane 4), GST-MKK4/SEK1 (lane 5), or GST-MKK5 (lane 6) bound to glutathione-agarose and analyzed as previously described ( 29,  30).	bind
1166	3	1416	5	10	NULL	0	NULL	YopJ	GP		bind		specifically			GST-MKK4/SEK1	GP	recombinant			NULL		NULL	NULL	NULL	NULL	gw60_science_285_5435_1920_s_35	10489373	( B) YopJ specifically bound recombinant GST-MKK1, GST-MKK3, GST-MKK4/SEK1, and GST-MKK5 but not GST. 35S-methionine-labeled pcDNA3-YopJ was incubated with bacterially expressed recombinant GST (lane 2), GST-MKK1 (lane 3), GST-MKK3 (lane 4), GST-MKK4/SEK1 (lane 5), or GST-MKK5 (lane 6) bound to glutathione-agarose and analyzed as previously described ( 29,  30).	bind
1167	4	1416	5	10	NULL	0	NULL	YopJ	GP		bind		specifically			GST-MKK5	GP	recombinant			NULL		NULL	NULL	NULL	NULL	gw60_science_285_5435_1920_s_35	10489373	( B) YopJ specifically bound recombinant GST-MKK1, GST-MKK3, GST-MKK4/SEK1, and GST-MKK5 but not GST. 35S-methionine-labeled pcDNA3-YopJ was incubated with bacterially expressed recombinant GST (lane 2), GST-MKK1 (lane 3), GST-MKK3 (lane 4), GST-MKK4/SEK1 (lane 5), or GST-MKK5 (lane 6) bound to glutathione-agarose and analyzed as previously described ( 29,  30).	bind
1169	5	1416	5	10	NULL	0	NULL	YopJ	GP		does not bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_285_5435_1920_s_35	10489373	( B) YopJ specifically bound recombinant GST-MKK1, GST-MKK3, GST-MKK4/SEK1, and GST-MKK5 but not GST. 35S-methionine-labeled pcDNA3-YopJ was incubated with bacterially expressed recombinant GST (lane 2), GST-MKK1 (lane 3), GST-MKK3 (lane 4), GST-MKK4/SEK1 (lane 5), or GST-MKK5 (lane 6) bound to glutathione-agarose and analyzed as previously described ( 29,  30).	bind
1431	1	1416	7	10	NULL	0	NULL	YopJ 	GP		bind		specifically			GST-MKK1	GP	recombinant 			NULL		NULL	NULL	NULL	NULL	gw60_science_285_5435_1920_s_35	10489373	( B) YopJ specifically bound recombinant GST-MKK1, GST-MKK3, GST-MKK4/SEK1, and GST-MKK5 but not GST. 35S-methionine-labeled pcDNA3-YopJ was incubated with bacterially expressed recombinant GST (lane 2), GST-MKK1 (lane 3), GST-MKK3 (lane 4), GST-MKK4/SEK1 (lane 5), or GST-MKK5 (lane 6) bound to glutathione-agarose and analyzed as previously described ( 29,  30).	bind
1432	2	1416	7	10	NULL	0	NULL	YopJ	GP		bind 		specifically			GST-MKK3	GP	recombinant			NULL		NULL	NULL	NULL	NULL	gw60_science_285_5435_1920_s_35	10489373	( B) YopJ specifically bound recombinant GST-MKK1, GST-MKK3, GST-MKK4/SEK1, and GST-MKK5 but not GST. 35S-methionine-labeled pcDNA3-YopJ was incubated with bacterially expressed recombinant GST (lane 2), GST-MKK1 (lane 3), GST-MKK3 (lane 4), GST-MKK4/SEK1 (lane 5), or GST-MKK5 (lane 6) bound to glutathione-agarose and analyzed as previously described ( 29,  30).	bind
1433	3	1416	7	10	NULL	0	NULL	YopJ	GP		bind		specifically			GST-MKK4/SEK1	GP	recombinant			NULL		NULL	NULL	NULL	NULL	gw60_science_285_5435_1920_s_35	10489373	( B) YopJ specifically bound recombinant GST-MKK1, GST-MKK3, GST-MKK4/SEK1, and GST-MKK5 but not GST. 35S-methionine-labeled pcDNA3-YopJ was incubated with bacterially expressed recombinant GST (lane 2), GST-MKK1 (lane 3), GST-MKK3 (lane 4), GST-MKK4/SEK1 (lane 5), or GST-MKK5 (lane 6) bound to glutathione-agarose and analyzed as previously described ( 29,  30).	bind
1434	4	1416	7	10	NULL	0	NULL	YopJ	GP		bind		specifically			GST-MKK5	GP	recombinant 			NULL		NULL	NULL	NULL	NULL	gw60_science_285_5435_1920_s_35	10489373	( B) YopJ specifically bound recombinant GST-MKK1, GST-MKK3, GST-MKK4/SEK1, and GST-MKK5 but not GST. 35S-methionine-labeled pcDNA3-YopJ was incubated with bacterially expressed recombinant GST (lane 2), GST-MKK1 (lane 3), GST-MKK3 (lane 4), GST-MKK4/SEK1 (lane 5), or GST-MKK5 (lane 6) bound to glutathione-agarose and analyzed as previously described ( 29,  30).	bind
1435	5	1416	7	10	NULL	0	NULL	YopJ	GP		does not bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_285_5435_1920_s_35	10489373	( B) YopJ specifically bound recombinant GST-MKK1, GST-MKK3, GST-MKK4/SEK1, and GST-MKK5 but not GST. 35S-methionine-labeled pcDNA3-YopJ was incubated with bacterially expressed recombinant GST (lane 2), GST-MKK1 (lane 3), GST-MKK3 (lane 4), GST-MKK4/SEK1 (lane 5), or GST-MKK5 (lane 6) bound to glutathione-agarose and analyzed as previously described ( 29,  30).	bind
1170	1	1417	5	10	NULL	0	NULL	ZapA	GP		bind					FtsZ	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_19_2544_s_191	12368265	( B) ZapA binds to FtsZ.	bind
1436	1	1417	7	10	NULL	0	NULL	ZapA	GP		bind					FtsZ	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_19_2544_s_191	12368265	( B) ZapA binds to FtsZ.	bind
1172	1	1418	5	NULL	NULL	0	NULL	[gamma-32]GTP-RhoV14	NULL		bind	NULL				GST	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_103_11_1561_s_232	10359565	( b) [gamma-32]GTP-RhoV14 bound to GST, GST-RhoGAP, and GST-IL-1Rcd was quantified by scintillation counting, and cpm bound to GST fusion proteins are normalized to those bound to GST in each of 7 independent experiments.	bind
1173	2	1418	5	NULL	NULL	0	NULL	[gamma-32]GTP-RhoV14	NULL		bind	NULL				GST-RhoGAP	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_103_11_1561_s_232	10359565	( b) [gamma-32]GTP-RhoV14 bound to GST, GST-RhoGAP, and GST-IL-1Rcd was quantified by scintillation counting, and cpm bound to GST fusion proteins are normalized to those bound to GST in each of 7 independent experiments.	bind
1174	3	1418	5	NULL	NULL	0	NULL	[gamma-32]GTP-RhoV14	NULL		bind	NULL				GST-IL-1Rcd	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_103_11_1561_s_232	10359565	( b) [gamma-32]GTP-RhoV14 bound to GST, GST-RhoGAP, and GST-IL-1Rcd was quantified by scintillation counting, and cpm bound to GST fusion proteins are normalized to those bound to GST in each of 7 independent experiments.	bind
1175	4	1418	5	NULL	NULL	0	NULL	cpm	NULL		bind	NULL				GST fusion proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_103_11_1561_s_232	10359565	( b) [gamma-32]GTP-RhoV14 bound to GST, GST-RhoGAP, and GST-IL-1Rcd was quantified by scintillation counting, and cpm bound to GST fusion proteins are normalized to those bound to GST in each of 7 independent experiments.	bind
1437	5	1418	7	NULL	NULL	0	NULL	[gamma-32]GTP-RhoV14	NULL		bind to	NULL				GST	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_103_11_1561_s_232	10359565	( b) [gamma-32]GTP-RhoV14 bound to GST, GST-RhoGAP, and GST-IL-1Rcd was quantified by scintillation counting, and cpm bound to GST fusion proteins are normalized to those bound to GST in each of 7 independent experiments.	bind
1438	6	1418	7	NULL	NULL	0	NULL	 [gamma-32]GTP-RhoV14	NULL		bind to	NULL				GST-RhoGAP	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_103_11_1561_s_232	10359565	( b) [gamma-32]GTP-RhoV14 bound to GST, GST-RhoGAP, and GST-IL-1Rcd was quantified by scintillation counting, and cpm bound to GST fusion proteins are normalized to those bound to GST in each of 7 independent experiments.	bind
1439	7	1418	7	NULL	NULL	0	NULL	[gamma-32]GTP-RhoV14 	NULL		bind to	NULL				GST-IL-1Rcd	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_103_11_1561_s_232	10359565	( b) [gamma-32]GTP-RhoV14 bound to GST, GST-RhoGAP, and GST-IL-1Rcd was quantified by scintillation counting, and cpm bound to GST fusion proteins are normalized to those bound to GST in each of 7 independent experiments.	bind
1588	8	1418	7	NULL	NULL	0	NULL	cpm	NULL		bind	NULL				GST fusion proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_103_11_1561_s_232	10359565	( b) [gamma-32]GTP-RhoV14 bound to GST, GST-RhoGAP, and GST-IL-1Rcd was quantified by scintillation counting, and cpm bound to GST fusion proteins are normalized to those bound to GST in each of 7 independent experiments.	bind
1177	1	1419	5	10	NULL	0	NULL	40S hnRNP proteins	GP		bind					DNase I	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_8_1725_s_167	11937625	( b,  e and  h) Western blot analyses of 40S hnRNP proteins bound to DNase I - Sepharose.	bind
1440	1	1419	7	10	NULL	0	NULL	40S-hnRNP proteins 	GP		bind					DNase I	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_8_1725_s_167	11937625	( b,  e and  h) Western blot analyses of 40S hnRNP proteins bound to DNase I - Sepharose.	bind
1178	1	1420	5	NULL	NULL	0	NULL	importin-GFP	NULL		bind	NULL				Pho4	NULL	WT	zz		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_17_2673_s_132	9732266	( B, C) (Lanes  1,5) About 3% of the importin-GFP loaded; (lanes  2,6) importin-GFP bound to Pho4WT-zz; (lanes  3,7) importin-GFP bound to Pho4delta157-164-zz; (lanes  4,8) importin-GFP bound to the IgG-Sepharose control.	bind
1179	8	1420	5	NULL	NULL	0	NULL	importin-GFP	NULL		bind	NULL				Pho4	NULL		delta157-164-zz		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_17_2673_s_132	9732266	( B, C) (Lanes  1,5) About 3% of the importin-GFP loaded; (lanes  2,6) importin-GFP bound to Pho4WT-zz; (lanes  3,7) importin-GFP bound to Pho4delta157-164-zz; (lanes  4,8) importin-GFP bound to the IgG-Sepharose control.	bind
1180	3	1420	5	NULL	NULL	0	NULL	importin-GFP	NULL		bind	NULL				IgG-Sepharose	NULL	control			NULL		0	NULL	NULL	NULL	gw60_genesdev_12_17_2673_s_132	9732266	( B, C) (Lanes  1,5) About 3% of the importin-GFP loaded; (lanes  2,6) importin-GFP bound to Pho4WT-zz; (lanes  3,7) importin-GFP bound to Pho4delta157-164-zz; (lanes  4,8) importin-GFP bound to the IgG-Sepharose control.	bind
1441	9	1420	7	NULL	NULL	0	NULL	 importin-GFP	NULL		bind to	NULL				Pho4	NULL	WT	zz		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_17_2673_s_132	9732266	( B, C) (Lanes  1,5) About 3% of the importin-GFP loaded; (lanes  2,6) importin-GFP bound to Pho4WT-zz; (lanes  3,7) importin-GFP bound to Pho4delta157-164-zz; (lanes  4,8) importin-GFP bound to the IgG-Sepharose control.	bind
1442	6	1420	7	NULL	NULL	0	NULL	importin-GFP	NULL		bind to	NULL				Pho4	NULL		delta157-164-zz		NULL		0	NULL	NULL	NULL	gw60_genesdev_12_17_2673_s_132	9732266	( B, C) (Lanes  1,5) About 3% of the importin-GFP loaded; (lanes  2,6) importin-GFP bound to Pho4WT-zz; (lanes  3,7) importin-GFP bound to Pho4delta157-164-zz; (lanes  4,8) importin-GFP bound to the IgG-Sepharose control.	bind
1443	7	1420	7	NULL	NULL	0	NULL	importin-GFP	NULL		bind to	NULL				IgG-Sepharose	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_17_2673_s_132	9732266	( B, C) (Lanes  1,5) About 3% of the importin-GFP loaded; (lanes  2,6) importin-GFP bound to Pho4WT-zz; (lanes  3,7) importin-GFP bound to Pho4delta157-164-zz; (lanes  4,8) importin-GFP bound to the IgG-Sepharose control.	bind
1181	1	1422	5	10	NULL	0	NULL	p130	GP	endogenous	bind					HDAC1	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_6_719_s_184	15769944	( B,C) Apoptotic stimuli lead to loss of cellular association between endogenous p130 and  HDAC1 ( B) or Suv39H1 ( C).	bind
1182	2	1422	5	10	NULL	0	NULL	p130	GP	endogenous	bind		alternately			Suv39H1	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_6_719_s_184	15769944	( B,C) Apoptotic stimuli lead to loss of cellular association between endogenous p130 and  HDAC1 ( B) or Suv39H1 ( C).	bind
1183	3	1422	5	10	NULL	0	NULL	apoptotic stimuli 	Process		leads to					statement 1	Process	loss of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_6_719_s_184	15769944	( B,C) Apoptotic stimuli lead to loss of cellular association between endogenous p130 and  HDAC1 ( B) or Suv39H1 ( C).	bind
1184	4	1422	5	10	NULL	0	NULL	apoptotic stimuli	Process		leads to					statement 2	Process	loss of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_6_719_s_184	15769944	( B,C) Apoptotic stimuli lead to loss of cellular association between endogenous p130 and  HDAC1 ( B) or Suv39H1 ( C).	bind
1444	1	1422	7	10	NULL	0	NULL	p130	GP	endogenous	associate					HDAC1	GP	cellular			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_6_719_s_184	15769944	( B,C) Apoptotic stimuli lead to loss of cellular association between endogenous p130 and  HDAC1 ( B) or Suv39H1 ( C).	bind
1445	2	1422	7	10	NULL	0	NULL	p130	GP	endogenous	associate					Suv39H1	GP	cellular			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_6_719_s_184	15769944	( B,C) Apoptotic stimuli lead to loss of cellular association between endogenous p130 and  HDAC1 ( B) or Suv39H1 ( C).	bind
1446	3	1422	7	10	NULL	0	NULL	Apoptotic stimuli	Process		lead to					statement 1	Process	loss of 			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_6_719_s_184	15769944	( B,C) Apoptotic stimuli lead to loss of cellular association between endogenous p130 and  HDAC1 ( B) or Suv39H1 ( C).	bind
1447	4	1422	7	10	NULL	0	NULL	Apoptotic stimuli	Process		lead to					statement 1	Process	loss of 			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_6_719_s_184	15769944	( B,C) Apoptotic stimuli lead to loss of cellular association between endogenous p130 and  HDAC1 ( B) or Suv39H1 ( C).	bind
1185	8	1424	5	NULL	NULL	0	NULL	TLE1	NULL	groucho family protein	bind	NULL				PRDI-BF1	NULL		repression domain		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_genesdev_13_1_125_s_175	9887105	( B,D) Groucho family proteins TLE1 and TLE2 bind to the repression domain of PRDI-BF1 in vitro.	bind
1186	9	1424	5	NULL	NULL	0	NULL	TLE2	NULL	groucho family protein	bind	NULL				PRDI-BF1	NULL		repression domain		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_genesdev_13_1_125_s_175	9887105	( B,D) Groucho family proteins TLE1 and TLE2 bind to the repression domain of PRDI-BF1 in vitro.	bind
1448	6	1424	7	NULL	NULL	0	NULL	TLE1	NULL	Groucho family proteins	bind to	NULL		 		PRDI-BF1	NULL		repression domain 		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_genesdev_13_1_125_s_175	9887105	( B,D) Groucho family proteins TLE1 and TLE2 bind to the repression domain of PRDI-BF1 in vitro.	bind
1449	7	1424	7	NULL	NULL	0	NULL	TLE2	NULL	Groucho family proteins	bind to	NULL				PRDI-BF1	NULL		repression domain 		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_genesdev_13_1_125_s_175	9887105	( B,D) Groucho family proteins TLE1 and TLE2 bind to the repression domain of PRDI-BF1 in vitro.	bind
1187	1	1425	5	10	NULL	0	NULL	Pcn1	GP	recombinant	bind					GST-Cdc27 proteins	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_19_5_1108_s_52	10698951	( B- D)  In vitro binding of recombinant Pcn1 to GST-Cdc27 proteins.	bind
1450	1	1425	7	10	NULL	0	NULL	Pcn1 	GP	recombinant	bind					GST-Cdc27 proteins	GP				NULL	In vitro	NULL	NULL	NULL	NULL	gw60_embo_19_5_1108_s_52	10698951	( B- D)  In vitro binding of recombinant Pcn1 to GST-Cdc27 proteins.	bind
1190	1	1426	5	NULL	NULL	0	NULL	PL	NULL	from CNC	quenched by	NULL				DNP-BS	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_1_49_s_38	11756675	( Ba) PL from CNC is quenched by DNP-BS  and recovered on the specific binding between DNP-BS  and anti-DNP antibody.	bind
1191	2	1426	5	NULL	NULL	0	NULL	DNP-BS	NULL		bind	NULL	specifically			anti-DNP antibody	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_1_49_s_38	11756675	( Ba) PL from CNC is quenched by DNP-BS  and recovered on the specific binding between DNP-BS  and anti-DNP antibody.	bind
1451	3	1426	7	NULL	NULL	0	NULL	DNP-BS 	NULL		bind	NULL	specific			anti-DNP antibody	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_1_49_s_38	11756675	( Ba) PL from CNC is quenched by DNP-BS  and recovered on the specific binding between DNP-BS  and anti-DNP antibody.	bind
1592	4	1426	7	NULL	NULL	0	NULL	PL	NULL	from CNC	quenched by	NULL				DNP-BS	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_1_49_s_38	11756675	( Ba) PL from CNC is quenched by DNP-BS  and recovered on the specific binding between DNP-BS  and anti-DNP antibody.	bind
1188	1	1427	5	10	NULL	0	NULL	Cbl-b protein	GP		bind					EGFR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_29_27677_s_154	11375397	( Bind  EGFR) shows the EGF-induced binding of each Cbl-b protein to the EGFR as determined by co-immunoprecipitation.	bind
1189	2	1427	5	10	NULL	0	NULL	EGF	GP		induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_29_27677_s_154	11375397	( Bind  EGFR) shows the EGF-induced binding of each Cbl-b protein to the EGFR as determined by co-immunoprecipitation.	bind
1452	1	1427	7	10	NULL	0	NULL	Cbl-b protein	GP		bind					EGFR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_29_27677_s_154	11375397	( Bind  EGFR) shows the EGF-induced binding of each Cbl-b protein to the EGFR as determined by co-immunoprecipitation.	bind
1453	2	1427	7	10	NULL	0	NULL	EGF	GP		induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_29_27677_s_154	11375397	( Bind  EGFR) shows the EGF-induced binding of each Cbl-b protein to the EGFR as determined by co-immunoprecipitation.	bind
1192	1	1428	5	10	NULL	0	NULL	Tfp	GP		bind					corneal epithelial cells	Cell	human			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_26_15276_s_107	11752467	( Bottom) Binding of Tfp to human corneal epithelial cells assesed by indirect immunofluorescence.	bind
1454	1	1428	7	10	NULL	0	NULL	Tfp	GP		bind 					corneal epithelial cells	Cell	human			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_26_15276_s_107	11752467	( Bottom) Binding of Tfp to human corneal epithelial cells assesed by indirect immunofluorescence.	bind
1193	1	1429	5	10	NULL	0	NULL	myosin	GP		bind		strongly			actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_47_16990_s_134	16287977	( Bottom) However, once a myosin binds strongly to actin, neighboring Tn - Tm regulatory units,  spanning three units, are activated, allowing myosins to bind at an accelerated rate  [ kwsx ( acc/ reg)].	bind
1194	2	1429	5	10	NULL	0	NULL	statement 1	Process		leads to					Tn - Tm regulatory units	GP	activation			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_47_16990_s_134	16287977	( Bottom) However, once a myosin binds strongly to actin, neighboring Tn - Tm regulatory units,  spanning three units, are activated, allowing myosins to bind at an accelerated rate  [ kwsx ( acc/ reg)].	bind
1195	3	1429	5	10	NULL	0	NULL	statement 2	Process		allows					myosin	GP	accelerated binding of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_47_16990_s_134	16287977	( Bottom) However, once a myosin binds strongly to actin, neighboring Tn - Tm regulatory units,  spanning three units, are activated, allowing myosins to bind at an accelerated rate  [ kwsx ( acc/ reg)].	bind
1455	1	1429	7	10	NULL	0	NULL	myosin	GP		bind		strongly			actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_47_16990_s_134	16287977	( Bottom) However, once a myosin binds strongly to actin, neighboring Tn - Tm regulatory units,  spanning three units, are activated, allowing myosins to bind at an accelerated rate  [ kwsx ( acc/ reg)].	bind
1456	2	1429	7	10	NULL	0	NULL	statement 1	Process		leads to					Tn - Tm regulatory units	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_47_16990_s_134	16287977	( Bottom) However, once a myosin binds strongly to actin, neighboring Tn - Tm regulatory units,  spanning three units, are activated, allowing myosins to bind at an accelerated rate  [ kwsx ( acc/ reg)].	bind
47957	3	1429	7	10	NULL	0	NULL	statement 2	Process		allows					myosin	GP	accelerated binding of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_47_16990_s_134	16287977	( Bottom) However, once a myosin binds strongly to actin, neighboring Tn - Tm regulatory units,  spanning three units, are activated, allowing myosins to bind at an accelerated rate  [ kwsx ( acc/ reg)].	bind
1196	1	1430	5	NULL	NULL	0	NULL	X2BP	NULL		bind	NULL	low affinity			NF-Y	NULL				NULL	RFX-deficient BLS cells	0	NULL	NULL	NULL	gw70_annurevimmunol_19_0_331_s_403	11244040	( Bottom) In RFX-deficient BLS cells, cooperative binding is lost, and the residual low binding  affinity of X2BP and NF-Y are not sufficient for stable promoter occupation in vivo.	bind
1549	2	1430	5	NULL	NULL	0	NULL	statement 1	NULL		is not sufficient for	NULL					NULL	stable occupation of		promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_annurevimmunol_19_0_331_s_403	11244040	( Bottom) In RFX-deficient BLS cells, cooperative binding is lost, and the residual low binding  affinity of X2BP and NF-Y are not sufficient for stable promoter occupation in vivo.	bind
1459	6	1430	7	NULL	NULL	0	NULL	X2BP	NULL		bind to	NULL	low affinity			NF-Y	NULL				NULL	in vivo in RFX-deficient BLS cells	NULL	NULL	NULL	NULL	gw70_annurevimmunol_19_0_331_s_403	11244040	( Bottom) In RFX-deficient BLS cells, cooperative binding is lost, and the residual low binding  affinity of X2BP and NF-Y are not sufficient for stable promoter occupation in vivo.	bind
1460	10	1430	7	NULL	NULL	0	NULL	statement 6	NULL		is not sufficient for	NULL					NULL	stable occupation of 		promoter	NULL	in vivo in RFX-deficient BLS cells	NULL	NULL	NULL	NULL	gw70_annurevimmunol_19_0_331_s_403	11244040	( Bottom) In RFX-deficient BLS cells, cooperative binding is lost, and the residual low binding  affinity of X2BP and NF-Y are not sufficient for stable promoter occupation in vivo.	bind
1241	1	1431	5	NULL	NULL	0	NULL	S3LC(2P)	NULL		bind	NULL				Ski	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_16_15_1950_s_190	12154125	( Bottom) S3LC(2P) binds Ski betterR than the unphosphorylated S3LC after extensive washing.	bind
1242	2	1431	5	NULL	NULL	0	NULL	S3LC	NULL	unphosphorylated	bind	NULL				Ski	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_16_15_1950_s_190	12154125	( Bottom) S3LC(2P) binds Ski betterR than the unphosphorylated S3LC after extensive washing.	bind
1243	3	1431	5	NULL	NULL	0	NULL	statement 1	NULL		better than	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_16_15_1950_s_190	12154125	( Bottom) S3LC(2P) binds Ski betterR than the unphosphorylated S3LC after extensive washing.	bind
1461	4	1431	7	NULL	NULL	0	NULL	S3LC(2P) 	NULL		binds	NULL				Ski 	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_16_15_1950_s_190	12154125	( Bottom) S3LC(2P) binds Ski betterR than the unphosphorylated S3LC after extensive washing.	bind
1462	5	1431	7	NULL	NULL	0	NULL	S3LC	NULL		binds 	NULL				 Ski	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_16_15_1950_s_190	12154125	( Bottom) S3LC(2P) binds Ski betterR than the unphosphorylated S3LC after extensive washing.	bind
1463	7	1431	7	NULL	NULL	0	NULL	statement 4	NULL		is better than 	NULL				statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_15_1950_s_190	12154125	( Bottom) S3LC(2P) binds Ski betterR than the unphosphorylated S3LC after extensive washing.	bind
1244	1	1434	5	10	NULL	0	NULL	CHC	GP		bind					p53	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_20_9_1087_s_180	16618797	( Bottom) The intensity of relative CHC binding to p53 was quantified by PhosphorImager.	bind
1464	1	1434	7	10	NULL	0	NULL	CHC	GP		bind					p53	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_20_9_1087_s_180	16618797	( Bottom) The intensity of relative CHC binding to p53 was quantified by PhosphorImager.	bind
1245	3	1435	5	NULL	NULL	0	NULL	tubby	NULL	putative transcription factor	bind	NULL	directly			PI(4,5)P2 phospholipid	NULL				NULL	in plasma membrane	NULL	NULL	NULL	NULL	gw60_science_292_5524_2019_s_25	11408644	( Bottom) The putative transcription factor tubby is directly bound to PI(4,5)P2, a phospholipid in the plasma membrane.	bind
1465	4	1435	7	NULL	NULL	0	NULL	tubby	NULL	putative transcription factor	bind to	NULL	directly			PI(4,5)P2 phospholipid	NULL				NULL	 in plasma membrane	NULL	NULL	NULL	NULL	gw60_science_292_5524_2019_s_25	11408644	( Bottom) The putative transcription factor tubby is directly bound to PI(4,5)P2, a phospholipid in the plasma membrane.	bind
1246	2	1436	5	NULL	NULL	0	NULL	Noxa	NULL	wild-type	bind	NULL				Mcl-1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_11_1294_s_172	15901672	( Bottom) Wild-type, but not mutant, Noxa bound Mcl-1 (fifth panel), disrupting the complex  between Mcl-1 and Bak.	bind
1247	3	1436	5	NULL	NULL	0	NULL	Noxa	NULL	mutant	does not bind	NULL				Mcl-1	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1294_s_172	15901672	( Bottom) Wild-type, but not mutant, Noxa bound Mcl-1 (fifth panel), disrupting the complex  between Mcl-1 and Bak.	bind
1248	4	1436	5	NULL	NULL	0	NULL	Mcl-1	NULL		bind	NULL				Bak	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1294_s_172	15901672	( Bottom) Wild-type, but not mutant, Noxa bound Mcl-1 (fifth panel), disrupting the complex  between Mcl-1 and Bak.	bind
1249	5	1436	5	NULL	NULL	0	NULL	statement 1	NULL		disrupt	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1294_s_172	15901672	( Bottom) Wild-type, but not mutant, Noxa bound Mcl-1 (fifth panel), disrupting the complex  between Mcl-1 and Bak.	bind
1466	6	1436	7	NULL	NULL	0	NULL	Noxa	NULL	Wild-type	bind to	NULL				Mcl-1	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1294_s_172	15901672	( Bottom) Wild-type, but not mutant, Noxa bound Mcl-1 (fifth panel), disrupting the complex  between Mcl-1 and Bak.	bind
1467	7	1436	7	NULL	NULL	0	NULL	Noxa	NULL	mutant	does not bind	NULL				Mcl-1	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1294_s_172	15901672	( Bottom) Wild-type, but not mutant, Noxa bound Mcl-1 (fifth panel), disrupting the complex  between Mcl-1 and Bak.	bind
1468	10	1436	7	NULL	NULL	0	NULL	Mcl-1	NULL		forms complex with	NULL				Bak	NULL				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_11_1294_s_172	15901672	( Bottom) Wild-type, but not mutant, Noxa bound Mcl-1 (fifth panel), disrupting the complex  between Mcl-1 and Bak.	bind
1469	11	1436	7	NULL	NULL	0	NULL	statement 6	NULL		disrupts	NULL				statement 10	NULL				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_11_1294_s_172	15901672	( Bottom) Wild-type, but not mutant, Noxa bound Mcl-1 (fifth panel), disrupting the complex  between Mcl-1 and Bak.	bind
49173	1	1439	5	10	NULL	0	NULL	GST - CBS1-4	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_113_2_274_s_105	14722619	( c and  d) Binding of AMP ( c) and ATP ( d) by the GST - CBS1-4 fusion proteins from gamma1, gamma2, and gamma3.	bind
49174	2	1439	5	10	NULL	0	NULL	GST - CBS1-4	GP		is obtained from					gamma1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_113_2_274_s_105	14722619	( c and  d) Binding of AMP ( c) and ATP ( d) by the GST - CBS1-4 fusion proteins from gamma1, gamma2, and gamma3.	bind
49175	3	1439	5	10	NULL	0	NULL	GST - CBS1-4	GP		is obtained from					gamma2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_113_2_274_s_105	14722619	( c and  d) Binding of AMP ( c) and ATP ( d) by the GST - CBS1-4 fusion proteins from gamma1, gamma2, and gamma3.	bind
49176	4	1439	5	10	NULL	0	NULL	GST - CBS1-4	GP		is obtained from					gamma3	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_113_2_274_s_105	14722619	( c and  d) Binding of AMP ( c) and ATP ( d) by the GST - CBS1-4 fusion proteins from gamma1, gamma2, and gamma3.	bind
49177	5	1439	5	10	NULL	0	NULL	AMP	Chemical		bind					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_113_2_274_s_105	14722619	( c and  d) Binding of AMP ( c) and ATP ( d) by the GST - CBS1-4 fusion proteins from gamma1, gamma2, and gamma3.	bind
49178	6	1439	5	10	NULL	0	NULL	AMP	Chemical		bind					statement 3	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_113_2_274_s_105	14722619	( c and  d) Binding of AMP ( c) and ATP ( d) by the GST - CBS1-4 fusion proteins from gamma1, gamma2, and gamma3.	bind
49179	7	1439	5	10	NULL	0	NULL	AMP	Chemical		bind					statement 4	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_113_2_274_s_105	14722619	( c and  d) Binding of AMP ( c) and ATP ( d) by the GST - CBS1-4 fusion proteins from gamma1, gamma2, and gamma3.	bind
49180	8	1439	5	10	NULL	0	NULL	ATP	Chemical		bind					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_113_2_274_s_105	14722619	( c and  d) Binding of AMP ( c) and ATP ( d) by the GST - CBS1-4 fusion proteins from gamma1, gamma2, and gamma3.	bind
49181	9	1439	5	10	NULL	0	NULL	ATP	Chemical		bind					statement 3	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_113_2_274_s_105	14722619	( c and  d) Binding of AMP ( c) and ATP ( d) by the GST - CBS1-4 fusion proteins from gamma1, gamma2, and gamma3.	bind
49182	10	1439	5	10	NULL	0	NULL	ATP	Chemical		bind					statement 4	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_113_2_274_s_105	14722619	( c and  d) Binding of AMP ( c) and ATP ( d) by the GST - CBS1-4 fusion proteins from gamma1, gamma2, and gamma3.	bind
1471	1	1439	7	10	NULL	0	NULL	GST - CBS1-4	GP		is obtained from					gamma1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_113_2_274_s_105	14722619	( c and  d) Binding of AMP ( c) and ATP ( d) by the GST - CBS1-4 fusion proteins from gamma1, gamma2, and gamma3.	bind
1472	2	1439	7	10	NULL	0	NULL	GST - CBS1-4	GP		is obtained from					gamma2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_113_2_274_s_105	14722619	( c and  d) Binding of AMP ( c) and ATP ( d) by the GST - CBS1-4 fusion proteins from gamma1, gamma2, and gamma3.	bind
1473	3	1439	7	10	NULL	0	NULL	GST - CBS1-4	GP		is obtained from					gamma3	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_113_2_274_s_105	14722619	( c and  d) Binding of AMP ( c) and ATP ( d) by the GST - CBS1-4 fusion proteins from gamma1, gamma2, and gamma3.	bind
1474	4	1439	7	10	NULL	0	NULL	GST - CBS1-4	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_113_2_274_s_105	14722619	( c and  d) Binding of AMP ( c) and ATP ( d) by the GST - CBS1-4 fusion proteins from gamma1, gamma2, and gamma3.	bind
48964	5	1439	7	10	NULL	0	NULL	AMP	Chemical		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_113_2_274_s_105	14722619	( c and  d) Binding of AMP ( c) and ATP ( d) by the GST - CBS1-4 fusion proteins from gamma1, gamma2, and gamma3.	bind
48965	6	1439	7	10	NULL	0	NULL	AMP	Chemical		bind					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_113_2_274_s_105	14722619	( c and  d) Binding of AMP ( c) and ATP ( d) by the GST - CBS1-4 fusion proteins from gamma1, gamma2, and gamma3.	bind
48966	7	1439	7	10	NULL	0	NULL	AMP	Chemical		bind					statement 3	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_113_2_274_s_105	14722619	( c and  d) Binding of AMP ( c) and ATP ( d) by the GST - CBS1-4 fusion proteins from gamma1, gamma2, and gamma3.	bind
48967	8	1439	7	10	NULL	0	NULL	ATP	Chemical		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_113_2_274_s_105	14722619	( c and  d) Binding of AMP ( c) and ATP ( d) by the GST - CBS1-4 fusion proteins from gamma1, gamma2, and gamma3.	bind
48968	9	1439	7	10	NULL	0	NULL	ATP	Chemical		bind					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_113_2_274_s_105	14722619	( c and  d) Binding of AMP ( c) and ATP ( d) by the GST - CBS1-4 fusion proteins from gamma1, gamma2, and gamma3.	bind
48969	10	1439	7	10	NULL	0	NULL	ATP	Chemical		bind					statement 3	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_113_2_274_s_105	14722619	( c and  d) Binding of AMP ( c) and ATP ( d) by the GST - CBS1-4 fusion proteins from gamma1, gamma2, and gamma3.	bind
1250	1	1442	5	10	NULL	0	NULL	Cy3-cAMP	Chemical		bind					Dictyostelium cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_science_294_5543_864_s_35	11679673	( C and  D) Fluorescence  images of Cy3-cAMP bound to  Dictyostelium cells.	bind
1476	2	1442	7	10	NULL	0	NULL	Cy3-cAMP	Chemical		bind					Dictyostelium cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_science_294_5543_864_s_35	11679673	( C and  D) Fluorescence  images of Cy3-cAMP bound to  Dictyostelium cells.	bind
1251	1	1443	5	10	NULL	0	NULL	pG3zf	GP		bind					BcrAbl probe	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_24_4865_s_107	11121477	( c and  d) Gel retardation assays of pG3zf and pG4zf binding the  BcrAbl probe in the presence of the  NonSp competitor.	bind
1252	2	1443	5	10	NULL	0	NULL	pG4zf	GP		bind					BcrAbl probe	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_24_4865_s_107	11121477	( c and  d) Gel retardation assays of pG3zf and pG4zf binding the  BcrAbl probe in the presence of the  NonSp competitor.	bind
1477	1	1443	7	10	NULL	0	NULL	pG3zf	GP		bind					BcrAbl probe	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_24_4865_s_107	11121477	( c and  d) Gel retardation assays of pG3zf and pG4zf binding the  BcrAbl probe in the presence of the  NonSp competitor.	bind
1478	2	1443	7	10	NULL	0	NULL	pG4zf	GP		bind					BcrAbl probe	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_24_4865_s_107	11121477	( c and  d) Gel retardation assays of pG3zf and pG4zf binding the  BcrAbl probe in the presence of the  NonSp competitor.	bind
1253	1	1445	5	10	NULL	0	NULL	GAPDH	GP		bind					Siah1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_10_3887_s_42	16505364	( c and  d) RAW264.7 cells were treated the same as in  b. ( c) TCH346 inhibits the binding of GAPDH and Siah1.	bind
1254	2	1445	5	10	NULL	0	NULL	TCH346	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_10_3887_s_42	16505364	( c and  d) RAW264.7 cells were treated the same as in  b. ( c) TCH346 inhibits the binding of GAPDH and Siah1.	bind
1479	1	1445	7	10	NULL	0	NULL	GAPDH	GP		bind 					Siah1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_10_3887_s_42	16505364	( c and  d) RAW264.7 cells were treated the same as in  b. ( c) TCH346 inhibits the binding of GAPDH and Siah1.	bind
1480	2	1445	7	10	NULL	0	NULL	TCH346	Chemical		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_10_3887_s_42	16505364	( c and  d) RAW264.7 cells were treated the same as in  b. ( c) TCH346 inhibits the binding of GAPDH and Siah1.	bind
1261	1	1446	5	NULL	NULL	0	NULL	LPC	NULL	isotherms of	bind	NULL				HEK293 G2A.GFP cells	NULL				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5530_702_s_60	11474113	( C and  D) Saturation isotherms of  [3]LPC and [3]SPC binding to HEK293  G2A.GFP cells.	bind
1263	2	1446	5	NULL	NULL	0	NULL	SPC	NULL	isotherms of	bind	NULL				HEK293 G2A.GFP cells	NULL				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5530_702_s_60	11474113	( C and  D) Saturation isotherms of  [3]LPC and [3]SPC binding to HEK293  G2A.GFP cells.	bind
1481	5	1446	7	NULL	NULL	0	NULL	[3]LPC	NULL	isotherms of 	bind to	NULL				HEK293 G2A.GFP cells	NULL				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5530_702_s_60	11474113	( C and  D) Saturation isotherms of  [3]LPC and [3]SPC binding to HEK293  G2A.GFP cells.	bind
1482	6	1446	7	NULL	NULL	0	NULL	[3]SPC	NULL	isotherms of	bind to	NULL				HEK293 G2A.GFP cells	NULL				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5530_702_s_60	11474113	( C and  D) Saturation isotherms of  [3]LPC and [3]SPC binding to HEK293  G2A.GFP cells.	bind
1264	1	1447	5	10	NULL	0	NULL	FGFR3c	GP		bind					heparin	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_4_935_s_205	14732692	( C and  D) Sensorgrams of the two-versus three-Ig form of FGFR3c binding to heparin.	bind
48904	1	1447	7	10	NULL	0	NULL	FGFR3c	GP		bind					heparin	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_4_935_s_205	14732692	( C and  D) Sensorgrams of the two-versus three-Ig form of FGFR3c binding to heparin.	bind
1265	1	1448	5	10	NULL	0	NULL	IP3R	GP	Purified;; full-length;; WT	bind					GAPDH	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_102_5_1357_s_55	15677321	( C Left) Purified full-length WT IP3R and GAPDH  in vitro binding demonstrated by Western analysis.	bind
1483	1	1448	7	10	NULL	0	NULL	IP3R	GP	Purified;; full-length;; WT	bind					GAPDH	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_102_5_1357_s_55	15677321	( C Left) Purified full-length WT IP3R and GAPDH  in vitro binding demonstrated by Western analysis.	bind
1266	1	1450	5	10	NULL	0	NULL	dCBP	GP		bind					Modulo	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_pnas_99_5_2895_s_99	11854460	( C)  In vitro binding between dCBP and Modulo.	bind
1484	1	1450	7	10	NULL	0	NULL	dCBP	GP		bind					Modulo	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_pnas_99_5_2895_s_99	11854460	( C)  In vitro binding between dCBP and Modulo.	bind
1267	1	1451	5	10	NULL	0	NULL	BRG1	GP		bind					HP1s	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_21_21_5797_s_64	12411497	( C)  In vitro binding of BRG1 to HP1s.	bind
1485	1	1451	7	10	NULL	0	NULL	BRG1	GP		bind					HP1s	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_21_21_5797_s_64	12411497	( C)  In vitro binding of BRG1 to HP1s.	bind
1268	1	1452	5	10	NULL	0	NULL	EF1gamma	GP		bind					Fez1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_pnas_98_18_10374_s_138	11504921	( C)  In vitro binding of EF1gamma to Fez1.	bind
1486	1	1452	7	10	NULL	0	NULL	EF1gamma	GP		bind					Fez1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_pnas_98_18_10374_s_138	11504921	( C)  In vitro binding of EF1gamma to Fez1.	bind
1269	1	1453	5	10	NULL	0	NULL	Mex67p	GP		bind					Yra1p	GP	GST-tagged			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_19_3_410_s_129	10722314	( C)  In vitro binding of Mex67p to GST-tagged Yra1p.	bind
1487	1	1453	7	10	NULL	0	NULL	Mex67p	GP		bind					Yra1p	GP	GST-tagged			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_19_3_410_s_129	10722314	( C)  In vitro binding of Mex67p to GST-tagged Yra1p.	bind
1270	1	1454	5	10	NULL	0	NULL	PalF	GP		bind					PalH	GP		cytoplasmic tail		NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_102_34_12141_s_94	16099830	( C)  In vitro binding of PalF to the PalH cytoplasmic tail.	bind
1488	1	1454	7	10	NULL	0	NULL	PalF 	GP		bind					PalH 	GP		cytoplasmic tail		NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_102_34_12141_s_94	16099830	( C)  In vitro binding of PalF to the PalH cytoplasmic tail.	bind
1271	1	1455	5	10	NULL	0	NULL	Rb	GP		bind					NS5B	GP	wt			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_102_50_18159_s_136	16332962	( C)  In vitro binding of Rb to wt and mutated NS5B.	bind
1272	2	1455	5	10	NULL	0	NULL	Rb	GP		bind					NS5B	GP	mutant			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_102_50_18159_s_136	16332962	( C)  In vitro binding of Rb to wt and mutated NS5B.	bind
1489	1	1455	7	10	NULL	0	NULL	Rb	GP		bind					NS5B	GP	wt			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_102_50_18159_s_136	16332962	( C)  In vitro binding of Rb to wt and mutated NS5B.	bind
1490	2	1455	7	10	NULL	0	NULL	Rb	GP		bind					NS5B	GP	mutant			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_102_50_18159_s_136	16332962	( C)  In vitro binding of Rb to wt and mutated NS5B.	bind
1273	1	1456	5	10	NULL	0	NULL	She2p	GP		bind					E2Bmin	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_102_50_18005_s_135	16326802	( c)  In vitro binding of She2p and She3p to E2Bmin.	bind
1274	2	1456	5	10	NULL	0	NULL	She3p	GP		bind					E2Bmin	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_102_50_18005_s_135	16326802	( c)  In vitro binding of She2p and She3p to E2Bmin.	bind
1491	1	1456	7	10	NULL	0	NULL	 She2p	GP		bind					 E2Bmin	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_102_50_18005_s_135	16326802	( c)  In vitro binding of She2p and She3p to E2Bmin.	bind
1492	2	1456	7	10	NULL	0	NULL	She3p	GP		bind 					E2Bmin	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_102_50_18005_s_135	16326802	( c)  In vitro binding of She2p and She3p to E2Bmin.	bind
1275	1	1457	5	10	NULL	0	NULL	MDM2	GP	in vitro-translated	bind					GST-RB	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_5_2211_s_127	11226218	( C)  In vitro-translated MDM2 binds to GST-RB and GST-Sp1.	bind
1276	2	1457	5	10	NULL	0	NULL	MDM2	GP	in vitro-translated	bind					GST-Sp1	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_5_2211_s_127	11226218	( C)  In vitro-translated MDM2 binds to GST-RB and GST-Sp1.	bind
1493	1	1457	7	10	NULL	0	NULL	MDM2	GP	In vitro-translated	bind					GST-RB	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_5_2211_s_127	11226218	( C)  In vitro-translated MDM2 binds to GST-RB and GST-Sp1.	bind
1494	2	1457	7	10	NULL	0	NULL	MDM2	GP	In vitro-translated	bind 					GST-Sp1	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_5_2211_s_127	11226218	( C)  In vitro-translated MDM2 binds to GST-RB and GST-Sp1.	bind
1277	1	1459	5	10	NULL	0	NULL	Pbs2	GP		bind					Ste11	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_embo_22_14_3624_s_145	12853477	( C)  In vivo binding of Pbs2 to Ste11.	bind
1495	1	1459	7	10	NULL	0	NULL	Pbs2	GP		bind					Ste11	GP				NULL	In vivo	NULL	NULL	NULL	NULL	gw60_embo_22_14_3624_s_145	12853477	( C)  In vivo binding of Pbs2 to Ste11.	bind
1278	1	1460	5	NULL	NULL	0	NULL	NF1	NULL	lipid-inhibited	bind	NULL				Ras GTP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_3_1566_s_230	8576154	( c)  Lipid-inhibited NF1 binds to Ras GTP propagating a signal through  NF1.	bind
2461	2	1460	5	NULL	NULL	0	NULL	signal	NULL		propagate through	NULL				NF1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_3_1566_s_230	8576154	( c)  Lipid-inhibited NF1 binds to Ras GTP propagating a signal through  NF1.	bind
2462	3	1460	5	NULL	NULL	0	NULL	statement 1	NULL		cause	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_3_1566_s_230	8576154	( c)  Lipid-inhibited NF1 binds to Ras GTP propagating a signal through  NF1.	bind
1604	2	1460	7	NULL	NULL	0	NULL	NF1	NULL	Lipid-inhibited	bind	NULL				Ras GTP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_3_1566_s_230	8576154	( c)  Lipid-inhibited NF1 binds to Ras GTP propagating a signal through  NF1.	bind
1605	3	1460	7	NULL	NULL	0	NULL	signal	NULL		propagate through	NULL				NF1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_3_1566_s_230	8576154	( c)  Lipid-inhibited NF1 binds to Ras GTP propagating a signal through  NF1.	bind
1924	4	1460	7	NULL	NULL	0	NULL	statement 2	NULL		cause	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_3_1566_s_230	8576154	( c)  Lipid-inhibited NF1 binds to Ras GTP propagating a signal through  NF1.	bind
1292	1	1464	5	10	NULL	0	NULL	RNase III	GP	S. aureus	bind		specifically			RNAIII	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_4_824_s_184	15678100	( C)  S. aureus RNase III binds specifically to RNAIII.	bind
1607	1	1464	7	10	NULL	0	NULL	RNase III	GP	S. aureus	bind		specifically			RNAIII	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_4_824_s_184	15678100	( C)  S. aureus RNase III binds specifically to RNAIII.	bind
1298	1	1465	5	10	NULL	0	NULL	actin	GP		bind					G6	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5446_1939_s_36	10583954	( C) (Left) Structure of the nonactivated G6 ( 4); (right) actin-bound form of G6 in a similar orientation.	bind
1758	1	1465	7	10	NULL	0	NULL	actin	GP		bind					G6	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5446_1939_s_36	10583954	( C) (Left) Structure of the nonactivated G6 ( 4); (right) actin-bound form of G6 in a similar orientation.	bind
1301	1	1468	5	10	NULL	0	NULL	9- Cis-4-oxo-RA	Chemical		bind					RARbeta-RXRalpha heterodimer	GP		 subunit		NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_26_15424_s_166	9860984	( C) 9- Cis-4-oxo-RA binds both subunits of RARbeta-RXRalpha heterodimers.	bind
1619	1	1468	7	10	NULL	0	NULL	9- Cis-4-oxo-RA	Chemical		bind					RARbeta-RXRalpha heterodimer	GP		 subunit		NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_26_15424_s_166	9860984	( C) 9- Cis-4-oxo-RA binds both subunits of RARbeta-RXRalpha heterodimers.	bind
1304	1	1469	5	NULL	NULL	0	NULL	GABAAR beta1 subunit	NULL	mutant	does not bind	NULL				BTX	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_54	16549768	( c) A GABAAR beta1 subunit that had been mutated to enhance its ability to form pentamers (beta1*) failed to bind BTX.	bind
2463	2	1469	5	NULL	NULL	0	NULL	GABAAR beta1	NULL	mutated	is enhanced for	NULL				pentamer beta1	NULL	formation of			NULL		0	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_54	16549768	( c) A GABAAR beta1 subunit that had been mutated to enhance its ability to form pentamers (beta1*) failed to bind BTX.	bind
1680	4	1469	7	NULL	NULL	0	NULL	GABAAR beta1	NULL	mutated	does not bind	NULL				BTX	NULL				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_54	16549768	( c) A GABAAR beta1 subunit that had been mutated to enhance its ability to form pentamers (beta1*) failed to bind BTX.	bind
1681	5	1469	7	NULL	NULL	0	NULL	GABAAR beta1	NULL	mutated	is enhanced for	NULL				pentamers beta1	NULL	formation of 			NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_54	16549768	( c) A GABAAR beta1 subunit that had been mutated to enhance its ability to form pentamers (beta1*) failed to bind BTX.	bind
1305	1	1470	5	10	NULL	0	NULL	CRK3	GP		bind					p13 suc1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_17_10153_s_233	9553063	( c) A putative inhibitor protein binds to the CRK3 kinase in metacyclic cells and interferes with the binding interaction between CRK3 and p13 suc1.	bind
1307	2	1470	5	10	NULL	0	NULL	inhibitor protein	GP	putative 	bind					CRK3 kinase	GP				NULL	metacyclic cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_17_10153_s_233	9553063	( c) A putative inhibitor protein binds to the CRK3 kinase in metacyclic cells and interferes with the binding interaction between CRK3 and p13 suc1.	bind
1309	3	1470	5	10	NULL	0	NULL	statement 2	Process		interferes with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_17_10153_s_233	9553063	( c) A putative inhibitor protein binds to the CRK3 kinase in metacyclic cells and interferes with the binding interaction between CRK3 and p13 suc1.	bind
1684	1	1470	7	10	NULL	0	NULL	inhibitor protein	GP	putative	bind					CRK3 kinase	GP				NULL	in metacyclic cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_17_10153_s_233	9553063	( c) A putative inhibitor protein binds to the CRK3 kinase in metacyclic cells and interferes with the binding interaction between CRK3 and p13 suc1.	bind
1685	2	1470	7	10	NULL	0	NULL	CRK3	GP		bind					p13 suc1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_17_10153_s_233	9553063	( c) A putative inhibitor protein binds to the CRK3 kinase in metacyclic cells and interferes with the binding interaction between CRK3 and p13 suc1.	bind
1686	3	1470	7	10	NULL	0	NULL	statement 1	Process		interferes with					statement 2 	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_17_10153_s_233	9553063	( c) A putative inhibitor protein binds to the CRK3 kinase in metacyclic cells and interferes with the binding interaction between CRK3 and p13 suc1.	bind
1311	1	1471	5	10	NULL	0	NULL			specific	bind			BRC repeat		RAD51	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_9_5287_s_130	9560268	( C) A specific BRC repeat binds to RAD51.	bind
1687	1	1471	7	10	NULL	0	NULL			specific	bind			BRC repeat		RAD51	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_9_5287_s_130	9560268	( C) A specific BRC repeat binds to RAD51.	bind
1312	1	1472	5	10	NULL	0	NULL	H22	GP		bind					S15	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_2_629_s_239	12527771	( C) A stereo view of the binding of H22 to S15.	bind
1688	1	1472	7	10	NULL	0	NULL	H22	GP		bind					S15	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_2_629_s_239	12527771	( C) A stereo view of the binding of H22 to S15.	bind
1313	1	1475	5	10	NULL	0	NULL	Ab	GP		bind					Abeta aggregates	GP		1-40		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_20_7115_s_99	15883377	( c) Ab binding to Abeta(1-40) aggregates.	bind
1689	1	1475	7	10	NULL	0	NULL	Ab	GP		bind					Abeta aggregates	GP		1-40		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_20_7115_s_99	15883377	( c) Ab binding to Abeta(1-40) aggregates.	bind
1314	1	1476	5	10	NULL	0	NULL	Cabin1	GP		bind					MEF2	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5440_790_s_99	10531067	( C) Activated CaM competes for Cabin1 binding with MEF2.	bind
1315	2	1476	5	10	NULL	0	NULL	CaM	GP	activated	bind					MEF2	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5440_790_s_99	10531067	( C) Activated CaM competes for Cabin1 binding with MEF2.	bind
2723	3	1476	5	10	NULL	0	NULL	statement 2	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5440_790_s_99	10531067	( C) Activated CaM competes for Cabin1 binding with MEF2.	bind
1690	1	1476	7	10	NULL	0	NULL	Cabin1	GP		bind					MEF2	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5440_790_s_99	10531067	( C) Activated CaM competes for Cabin1 binding with MEF2.	bind
1691	2	1476	7	10	NULL	0	NULL	CaM	GP	Activated	bind					MEF2	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5440_790_s_99	10531067	( C) Activated CaM competes for Cabin1 binding with MEF2.	bind
1925	3	1476	7	10	NULL	0	NULL	statement 2	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5440_790_s_99	10531067	( C) Activated CaM competes for Cabin1 binding with MEF2.	bind
1316	1	1477	5	10	NULL	0	NULL	Adipophilin	GP		does not bind					Rab9	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_11_7450_s_142	12032303	( C) Adipophilin does not bind Rab9.	bind
1692	1	1477	7	10	NULL	0	NULL	Adipophilin 	GP		does not bind					Rab9	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_11_7450_s_142	12032303	( C) Adipophilin does not bind Rab9.	bind
1317	1	1478	5	10	NULL	0	NULL	spORC	GP		bind					ars1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_52_17952_s_168	15598736	( C) AFM images of spORC and spOrc4p bound to  ars1.	bind
1318	2	1478	5	10	NULL	0	NULL	spOrc4p	GP		bind					ars1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_52_17952_s_168	15598736	( C) AFM images of spORC and spOrc4p bound to  ars1.	bind
1693	1	1478	7	10	NULL	0	NULL	spORC	GP		bind					ars1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_52_17952_s_168	15598736	( C) AFM images of spORC and spOrc4p bound to  ars1.	bind
1694	2	1478	7	10	NULL	0	NULL	spOrc4p	GP		bind					ars1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_52_17952_s_168	15598736	( C) AFM images of spORC and spOrc4p bound to  ars1.	bind
1319	1	1481	5	NULL	NULL	0	NULL	HrcQB	NULL		bind	NULL				His-10-HrcQA protein	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_101_1_70_s_136	14694203	( C) An autoradiogram that shows the binding of HrcQB to His-10-HrcQA protein and to the C-terminal truncated version.	bind
1320	2	1481	5	NULL	NULL	0	NULL	HrcQB	NULL		bind	NULL				His-10-HrcQA protein	NULL		C-terminal truncated version		NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_1_70_s_136	14694203	( C) An autoradiogram that shows the binding of HrcQB to His-10-HrcQA protein and to the C-terminal truncated version.	bind
1695	3	1481	7	NULL	NULL	0	NULL	HrcQB	NULL		bind to	NULL				His-10-HrcQA	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_101_1_70_s_136	14694203	( C) An autoradiogram that shows the binding of HrcQB to His-10-HrcQA protein and to the C-terminal truncated version.	bind
1696	4	1481	7	NULL	NULL	0	NULL	HrcQB	NULL		bind to	NULL				His-10-HrcQA	NULL		C-terminal truncated version		NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_1_70_s_136	14694203	( C) An autoradiogram that shows the binding of HrcQB to His-10-HrcQA protein and to the C-terminal truncated version.	bind
1321	1	1482	5	10	NULL	0	NULL	Cry11Aa toxin	GP		bind					Cyt1Aa	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_51_18303_s_216	16339907	( C) Analysis of binding of Cry11Aa toxin to Cyt1Aa by ELISA in the presence or absence  of 10 - 100 M excess of synthetic peptides corresponding to the loops and exposed  regions of Cry11Aa-domain II.	bind
1697	1	1482	7	10	NULL	0	NULL	Cry11Aa toxin	GP		bind					Cyt1Aa	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_51_18303_s_216	16339907	( C) Analysis of binding of Cry11Aa toxin to Cyt1Aa by ELISA in the presence or absence  of 10 - 100 M excess of synthetic peptides corresponding to the loops and exposed  regions of Cry11Aa-domain II.	bind
1322	1	1483	5	10	NULL	0	NULL	Tat	GP	HIV-1	bind					TAR RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_22_3512_s_187	9832504	( C) Analysis of the ability of murine CycT1 to enhance the binding of HIV-1 Tat to TAR RNA.	bind
1323	2	1483	5	10	NULL	0	NULL	CycT1	GP	murine	enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_22_3512_s_187	9832504	( C) Analysis of the ability of murine CycT1 to enhance the binding of HIV-1 Tat to TAR RNA.	bind
1699	1	1483	7	10	NULL	0	NULL	 Tat 	GP	HIV-1	bind					TAR RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_22_3512_s_187	9832504	( C) Analysis of the ability of murine CycT1 to enhance the binding of HIV-1 Tat to TAR RNA.	bind
1700	2	1483	7	10	NULL	0	NULL	CycT1 	GP	murine	enhance					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_22_3512_s_187	9832504	( C) Analysis of the ability of murine CycT1 to enhance the binding of HIV-1 Tat to TAR RNA.	bind
1324	1	1484	5	10	NULL	0	NULL	APA1/1 antibody	GP		bind					TCR	GP				NULL	in the cortex of the thymus	NULL	NULL	NULL	NULL	gw70_pnas_103_25_9625_s_57	16766661	( C) APA1/1 antibody binds to the TCR in the cortex of the thymus but not in the medulla.	bind
46523	2	1484	5	10	NULL	0	NULL	APA1/1 antibody	GP		does not bind					TCR	GP				NULL	medulla of thymus	NULL	NULL	NULL	NULL	gw70_pnas_103_25_9625_s_57	16766661	( C) APA1/1 antibody binds to the TCR in the cortex of the thymus but not in the medulla.	bind
1701	1	1484	7	10	NULL	0	NULL	APA1/1 antibody	GP		bind					TCR	GP				NULL	in the cortex of the thymus	NULL	NULL	NULL	NULL	gw70_pnas_103_25_9625_s_57	16766661	( C) APA1/1 antibody binds to the TCR in the cortex of the thymus but not in the medulla.	bind
1702	2	1484	7	10	NULL	0	NULL	APA1/1 antibody	GP		does not bind 					TCR	GP				NULL	medulla of thymus	NULL	NULL	NULL	NULL	gw70_pnas_103_25_9625_s_57	16766661	( C) APA1/1 antibody binds to the TCR in the cortex of the thymus but not in the medulla.	bind
1325	1	1485	5	10	NULL	0	NULL	tubulin	GP	bovine	bind					GST-Aut2p glutathione-Sepharose 4B	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_13_3597_s_134	9649430	( C) As described in (B), bovine tubulin binds to GST-Aut2p glutathione-Sepharose 4B (lane 12), but not to GST glutathione-Sepharose 4B (lane 9).	bind
1326	2	1485	5	10	NULL	0	NULL	tubulin	GP	bovine	does not bind					GST glutathione-Sepharose 4B	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_13_3597_s_134	9649430	( C) As described in (B), bovine tubulin binds to GST-Aut2p glutathione-Sepharose 4B (lane 12), but not to GST glutathione-Sepharose 4B (lane 9).	bind
1703	1	1485	7	10	NULL	0	NULL	tubulin 	GP	bovine	bind					GST-Aut2p glutathione-Sepharose 4B	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_13_3597_s_134	9649430	( C) As described in (B), bovine tubulin binds to GST-Aut2p glutathione-Sepharose 4B (lane 12), but not to GST glutathione-Sepharose 4B (lane 9).	bind
1704	2	1485	7	10	NULL	0	NULL	tubulin 	GP	bovine	does not bind					GST glutathione-Sepharose 4B 	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_13_3597_s_134	9649430	( C) As described in (B), bovine tubulin binds to GST-Aut2p glutathione-Sepharose 4B (lane 12), but not to GST glutathione-Sepharose 4B (lane 9).	bind
1334	1	1486	5	10	NULL	0	NULL	Par6	GP		bind					Cdc42	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_22_5_1125_s_83	12606577	( C) Asp38 is not required for binding of Par6 to Cdc42.	bind
1335	2	1486	5	10	NULL	0	NULL				is not required for			Asp38		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_22_5_1125_s_83	12606577	( C) Asp38 is not required for binding of Par6 to Cdc42.	bind
1705	1	1486	7	10	NULL	0	NULL	Par6 	GP		bind 					Cdc42	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_22_5_1125_s_83	12606577	( C) Asp38 is not required for binding of Par6 to Cdc42.	bind
1706	2	1486	7	10	NULL	0	NULL				is not required for			Asp38		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_22_5_1125_s_83	12606577	( C) Asp38 is not required for binding of Par6 to Cdc42.	bind
1344	1	1488	5	10	NULL	0	NULL	1alpha,25(OH)2D3	Chemical		bind					VDR	GP		LBD		NULL		NULL	NULL	NULL	NULL	gw60_embo_21_22_5960_s_80	12426368	( C) Atomic model of 1alpha,25(OH)2D3 bound to the VDR LBD ( Rochel  et al., 2000; PDB code 1DB1).	bind
1708	1	1488	7	10	NULL	0	NULL	1alpha,25(OH)2D3	Chemical		bind 					VDR	GP		LBD		NULL		NULL	NULL	NULL	NULL	gw60_embo_21_22_5960_s_80	12426368	( C) Atomic model of 1alpha,25(OH)2D3 bound to the VDR LBD ( Rochel  et al., 2000; PDB code 1DB1).	bind
1350	1	1489	5	10	NULL	0	NULL	DnaB	GP	32P-labeled	bind					Tus-GST	GP	wt			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_17_9569_s_141	11493686	( C) Autoradiogram showing the binding of 32P-labeled DnaB to wt and mutant form of Tus-GST affinity matrices and the lack of binding of labeled DnaG to the wt Tus-GST matrix.	bind
1352	2	1489	5	10	NULL	0	NULL	DnaB	GP	32P-labeled	bind					Tus-GST	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_17_9569_s_141	11493686	( C) Autoradiogram showing the binding of 32P-labeled DnaB to wt and mutant form of Tus-GST affinity matrices and the lack of binding of labeled DnaG to the wt Tus-GST matrix.	bind
1353	3	1489	5	10	NULL	0	NULL	DnaG	GP	labeled	does not bind					Tus-GST	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_17_9569_s_141	11493686	( C) Autoradiogram showing the binding of 32P-labeled DnaB to wt and mutant form of Tus-GST affinity matrices and the lack of binding of labeled DnaG to the wt Tus-GST matrix.	bind
1709	1	1489	7	10	NULL	0	NULL	 DnaB	GP	32P-labeled	bind 					Tus-GST	GP	wt 			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_17_9569_s_141	11493686	( C) Autoradiogram showing the binding of 32P-labeled DnaB to wt and mutant form of Tus-GST affinity matrices and the lack of binding of labeled DnaG to the wt Tus-GST matrix.	bind
1710	2	1489	7	10	NULL	0	NULL	DnaB	GP	32P-labeled 	bind					Tus-GST	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_17_9569_s_141	11493686	( C) Autoradiogram showing the binding of 32P-labeled DnaB to wt and mutant form of Tus-GST affinity matrices and the lack of binding of labeled DnaG to the wt Tus-GST matrix.	bind
1711	3	1489	7	10	NULL	0	NULL	 DnaG	GP	labeled	does not bind					Tus-GST 	GP	wt			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_17_9569_s_141	11493686	( C) Autoradiogram showing the binding of 32P-labeled DnaB to wt and mutant form of Tus-GST affinity matrices and the lack of binding of labeled DnaG to the wt Tus-GST matrix.	bind
1358	1	1490	5	10	NULL	0	NULL	BC1/BC200	GP		bind					PABP	GP		adenine-rich region		NULL		NULL	NULL	NULL	NULL	gw70_annurevneurosci_29_0_77_s_310	16776580	( C) BC1/BC200 bind to PABP through an adenine-rich region, titrating PABP and possibly  other initiation factors away from mRNAs and thus inhibiting translation.	bind
1712	1	1490	7	10	NULL	0	NULL	BC1/BC200	GP		bind					PABP 	GP		adenine-rich region		NULL		NULL	NULL	NULL	NULL	gw70_annurevneurosci_29_0_77_s_310	16776580	( C) BC1/BC200 bind to PABP through an adenine-rich region, titrating PABP and possibly  other initiation factors away from mRNAs and thus inhibiting translation.	bind
1360	1	1491	5	10	NULL	0	NULL	beta-NAD+	Chemical		bind					TRPM2 fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_9_1804_s_82	16601673	( C) beta-NAD+ binding to the TRPM2 fusion proteins in the presence (+) or absence (-) of cADPR.	bind
1715	1	1491	7	10	NULL	0	NULL	 beta-NAD+	Chemical		bind 					TRPM2 fusion proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_9_1804_s_82	16601673	( C) beta-NAD+ binding to the TRPM2 fusion proteins in the presence (+) or absence (-) of cADPR.	bind
1361	1	1492	5	10	NULL	0	NULL	 B. pertussis	Organism		bind					mucin-coated plates	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_25_13847_s_160	11087813	( c) Binding of  B. pertussis to mucin-coated plates.	bind
1713	2	1492	7	10	NULL	0	NULL	B. pertussis	Organism		bind 					mucin-coated plates	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_25_13847_s_160	11087813	( c) Binding of  B. pertussis to mucin-coated plates.	bind
1363	1	1493	5	10	NULL	0	NULL	Af-SRP19	GP		bind					SRP RNAs	NucleicAcid	various			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_6_1365_s_159	10684931	( C) Binding of Af-SRP19 and Af-SRP54 to various SRP RNAs.	bind
1364	2	1493	5	10	NULL	0	NULL	Af-SRP54	GP		bind					SRP RNAs	NucleicAcid	various			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_6_1365_s_159	10684931	( C) Binding of Af-SRP19 and Af-SRP54 to various SRP RNAs.	bind
1716	1	1493	7	10	NULL	0	NULL	Af-SRP19	GP		bind					SRP RNAs	NucleicAcid	various			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_6_1365_s_159	10684931	( C) Binding of Af-SRP19 and Af-SRP54 to various SRP RNAs.	bind
1717	5	1493	7	10	NULL	0	NULL	Af-SRP54	GP		bind					SRP RNAs	NucleicAcid	various			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_6_1365_s_159	10684931	( C) Binding of Af-SRP19 and Af-SRP54 to various SRP RNAs.	bind
1365	1	1495	5	NULL	NULL	0	NULL	anti-C1q autoantibodies	NULL		bind	NULL				C1q	NULL				NULL	present on the immune complexes	NULL	NULL	NULL	NULL	gw70_jclininvest_114_5_679_s_223	15343386	( C) Binding of anti-C1q autoantibodies to C1q present on the immune complexes.	bind
1718	2	1495	7	NULL	NULL	0	NULL	anti-C1q autoantibodies	NULL		bind to	NULL				C1q 	NULL				NULL	present on the immune complexes	0	NULL	NULL	NULL	gw70_jclininvest_114_5_679_s_223	15343386	( C) Binding of anti-C1q autoantibodies to C1q present on the immune complexes.	bind
1366	1	1496	5	10	NULL	0	NULL	B cells	Cell		bind					PtC liposomes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_23_13459_s_142	14595020	( C) Binding of B cells to PtC liposomes.	bind
1719	1	1496	7	10	NULL	0	NULL	B cells	Cell		bind					PtC liposomes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_23_13459_s_142	14595020	( C) Binding of B cells to PtC liposomes.	bind
1367	1	1497	5	NULL	NULL	0	NULL	CBFA1	NULL		bind	NULL				OSE2 oligonucleotide	NULL				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_9_2254_s_265	11331591	( C) Binding of CBFA1 to an OSE2 oligonucleotide, in the absence or presence of equimolar levels of Smad3 and Smad4.	bind
1720	3	1497	7	NULL	NULL	0	NULL	CBFA1	NULL		bind to	NULL				OSE2 oligonucleotide	NULL				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_9_2254_s_265	11331591	( C) Binding of CBFA1 to an OSE2 oligonucleotide, in the absence or presence of equimolar levels of Smad3 and Smad4.	bind
1368	1	1498	5	10	NULL	0	NULL	IgA	GP		bind					R1 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_105_12_1731_s_173	10862788	( c) Binding of control IgA and T15 to R1 cells.	bind
1369	2	1498	5	10	NULL	0	NULL	T15	GP		bind					R1 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_105_12_1731_s_173	10862788	( c) Binding of control IgA and T15 to R1 cells.	bind
1724	1	1498	7	10	NULL	0	NULL	IgA	GP		bind					R1 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_105_12_1731_s_173	10862788	( c) Binding of control IgA and T15 to R1 cells.	bind
1725	2	1498	7	10	NULL	0	NULL	T15	GP		bind 					R1 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_105_12_1731_s_173	10862788	( c) Binding of control IgA and T15 to R1 cells.	bind
1370	1	1499	5	10	NULL	0	NULL	Crb2	GP		bind					Cut5	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_genesdev_11_24_3387_s_85	9407031	( C) Binding of Crb2 and Crb3 with Cut5 in vitro.	bind
1371	2	1499	5	10	NULL	0	NULL	Crb3	GP		bind					Cut5	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_genesdev_11_24_3387_s_85	9407031	( C) Binding of Crb2 and Crb3 with Cut5 in vitro.	bind
1726	1	1499	7	10	NULL	0	NULL	Crb2	GP		bind					Cut5	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_genesdev_11_24_3387_s_85	9407031	( C) Binding of Crb2 and Crb3 with Cut5 in vitro.	bind
1727	2	1499	7	10	NULL	0	NULL	Crb3	GP		bind					Cut5	GP				NULL	 in vitro	NULL	NULL	NULL	NULL	gw60_genesdev_11_24_3387_s_85	9407031	( C) Binding of Crb2 and Crb3 with Cut5 in vitro.	bind
1372	1	1500	5	NULL	NULL	0	NULL	DHE	NULL		bind	NULL				NPC2	NULL				NULL	at pH 5 and 7	0	NULL	NULL	NULL	gw60_pnas_100_5_2512_s_88	12591954	( C) Binding of DHE to NPC2 at pH 5 and 7.	bind
1728	2	1500	7	NULL	NULL	0	NULL	DHE	NULL		bind to	NULL				NPC2	NULL				NULL	at pH 5	0	NULL	NULL	NULL	gw60_pnas_100_5_2512_s_88	12591954	( C) Binding of DHE to NPC2 at pH 5 and 7.	bind
1729	3	1500	7	NULL	NULL	0	NULL	DHE	NULL		bind to	NULL				NPC2	NULL				NULL	at pH 7	0	NULL	NULL	NULL	gw60_pnas_100_5_2512_s_88	12591954	( C) Binding of DHE to NPC2 at pH 5 and 7.	bind
1373	1	1501	5	NULL	NULL	0	NULL	EIL proteins	NULL		bind	NULL				ERF1	NULL			EIN3 target site in promoter	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_23_3703_s_84	9851977	( C) Binding of EIL proteins to the EIN3 target site in the  ERF1 promoter.	bind
1730	2	1501	7	NULL	NULL	0	NULL	EIL proteins	NULL		bind to	NULL				ERF1	NULL			EIN3 target site in the promoter of 	NULL		0	NULL	NULL	NULL	gw60_genesdev_12_23_3703_s_84	9851977	( C) Binding of EIL proteins to the EIN3 target site in the  ERF1 promoter.	bind
1374	1	1502	5	NULL	NULL	0	NULL	GluR2/3	NULL	endogenous	bind	NULL				GRIP1aHA	NULL	overexpressed			NULL		0	NULL	NULL	NULL	gw70_embo_24_18_3266_s_188	16138078	( C) Binding of endogenous GluR2/3 to overexpressed GRIP1aHA is not Ca2+-sensitive.	bind
1375	2	1502	5	NULL	NULL	0	NULL	statement 1	NULL		is not sensitive to	NULL				Ca2+	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_24_18_3266_s_188	16138078	( C) Binding of endogenous GluR2/3 to overexpressed GRIP1aHA is not Ca2+-sensitive.	bind
1731	3	1502	7	NULL	NULL	0	NULL	GluR2/3	NULL	endogenous	bind to	NULL				GRIP1aHA	NULL	overexpressed			NULL		0	NULL	NULL	NULL	gw70_embo_24_18_3266_s_188	16138078	( C) Binding of endogenous GluR2/3 to overexpressed GRIP1aHA is not Ca2+-sensitive.	bind
1732	4	1502	7	NULL	NULL	0	NULL	statement 3	NULL		is not sensitive to	NULL				Ca2+	NULL				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_18_3266_s_188	16138078	( C) Binding of endogenous GluR2/3 to overexpressed GRIP1aHA is not Ca2+-sensitive.	bind
1376	1	1503	5	NULL	NULL	0	NULL	gp4	NULL		bind	NULL				flow cells	NULL				NULL	containing gp5/trx - primer/template	NULL	NULL	NULL	NULL	gw70_pnas_102_14_5096_s_183	15795374	( C) Binding of gp4 and gp4-Cdelta17 to flow cells containing the gp5/trx - primer/template in the two orientations  shown in  A.	bind
1377	2	1503	5	NULL	NULL	0	NULL	gp4-Cdelta17	NULL		bind	NULL				flow cells	NULL				NULL	containing gp5/trx - primer/template	NULL	NULL	NULL	NULL	gw70_pnas_102_14_5096_s_183	15795374	( C) Binding of gp4 and gp4-Cdelta17 to flow cells containing the gp5/trx - primer/template in the two orientations  shown in  A.	bind
1733	4	1503	7	NULL	NULL	0	NULL	gp4	NULL		bind to	NULL				flow cells	NULL				NULL	containing the gp5/trx - primer/template	NULL	NULL	NULL	NULL	gw70_pnas_102_14_5096_s_183	15795374	( C) Binding of gp4 and gp4-Cdelta17 to flow cells containing the gp5/trx - primer/template in the two orientations  shown in  A.	bind
1735	6	1503	7	NULL	NULL	0	NULL	gp4-Cdelta17	NULL		bind to	NULL				flow cells	NULL				NULL	containing the gp5/trx - primer/template	NULL	NULL	NULL	NULL	gw70_pnas_102_14_5096_s_183	15795374	( C) Binding of gp4 and gp4-Cdelta17 to flow cells containing the gp5/trx - primer/template in the two orientations  shown in  A.	bind
1378	1	1504	5	10	NULL	0	NULL	GST-Rsp5 proteins	GP		bind					Ubp2	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_13_2414_s_125	15933713	( C) Binding of GST-Rsp5 proteins to Ubp2.	bind
1737	1	1504	7	10	NULL	0	NULL	GST-Rsp5 proteins	GP		bind					Ubp2	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_13_2414_s_125	15933713	( C) Binding of GST-Rsp5 proteins to Ubp2.	bind
1379	1	1505	5	NULL	NULL	0	NULL	GST-Rsp5	NULL		bind	NULL				Ubp2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_13_2414_s_137	15933713	( C) Binding of GST-Rsp5 to Ubp2, in the presence of Rup1.	bind
1550	2	1505	5	NULL	NULL	0	NULL	statement 1	NULL		in the presence of	NULL				Rup1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_13_2414_s_137	15933713	( C) Binding of GST-Rsp5 to Ubp2, in the presence of Rup1.	bind
1738	3	1505	7	NULL	NULL	0	NULL	GST-Rsp5	NULL		bind to	NULL				Ubp2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_13_2414_s_137	15933713	( C) Binding of GST-Rsp5 to Ubp2, in the presence of Rup1.	bind
2206	4	1505	7	NULL	NULL	0	NULL	statement 3	NULL		in the presence of 	NULL				Rup1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_13_2414_s_137	15933713	( C) Binding of GST-Rsp5 to Ubp2, in the presence of Rup1.	bind
1380	1	1506	5	10	NULL	0	NULL	HCV	GP		bind					CD81	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_282_5390_938_s_77	9794763	( C) Binding of HCV to CD81.	bind
1739	1	1506	7	10	NULL	0	NULL	HCV	GP		bind 					CD81	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_282_5390_938_s_77	9794763	( C) Binding of HCV to CD81.	bind
1381	1	1507	5	10	NULL	0	NULL	histone H4	GP		bind					UBC9	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_23_13225_s_101	14578449	( C) Binding of histone H4 to UBC9.	bind
1740	1	1507	7	10	NULL	0	NULL	histone H4	GP		bind					UBC9	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_23_13225_s_101	14578449	( C) Binding of histone H4 to UBC9.	bind
1383	1	1508	5	10	NULL	0	NULL	mad2 gene product	GP	in vitro-translated;;35S labeled	bind					GST-Slp1 fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_279_5353_1045_s_37	9461438	( C) Binding of in vitro-translated  mad2 gene product labeled by 35S (lane 1) to GST protein or a fusion protein, GST-Slp1, which were bound to glutathione-Sepharose 4B beads.	bind
1743	1	1508	7	10	NULL	0	NULL	mad2 gene product	GP	in vitro-translated;;35S labeled	bind					GST-Slp1 fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_279_5353_1045_s_37	9461438	( C) Binding of in vitro-translated  mad2 gene product labeled by 35S (lane 1) to GST protein or a fusion protein, GST-Slp1, which were bound to glutathione-Sepharose 4B beads.	bind
1384	1	1509	5	10	NULL	0	NULL				bind			catalytic IDH2 site		isocitrate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_15_12864_s_270	12562755	( C) Binding of isocitrate by the catalytic IDH2 site, but not by the regulatory IDH1 site, requires Mg2+.	bind
1385	2	1509	5	10	NULL	0	NULL	statement 1	Process		require					Mg2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_15_12864_s_270	12562755	( C) Binding of isocitrate by the catalytic IDH2 site, but not by the regulatory IDH1 site, requires Mg2+.	bind
1386	3	1509	5	10	NULL	0	NULL				does not bind			regulatory IDH1 site		isocitrate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_15_12864_s_270	12562755	( C) Binding of isocitrate by the catalytic IDH2 site, but not by the regulatory IDH1 site, requires Mg2+.	bind
1744	1	1509	7	10	NULL	0	NULL	isocitrate	Chemical		bind to 								catalytic IDH2 site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_15_12864_s_270	12562755	( C) Binding of isocitrate by the catalytic IDH2 site, but not by the regulatory IDH1 site, requires Mg2+.	bind
1745	2	1509	7	10	NULL	0	NULL	isocitrate	Chemical		does not bind								regulatory IDH1 site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_15_12864_s_270	12562755	( C) Binding of isocitrate by the catalytic IDH2 site, but not by the regulatory IDH1 site, requires Mg2+.	bind
1746	3	1509	7	10	NULL	0	NULL	statement 1	Process		requires					Mg2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_15_12864_s_270	12562755	( C) Binding of isocitrate by the catalytic IDH2 site, but not by the regulatory IDH1 site, requires Mg2+.	bind
1387	1	1510	5	10	NULL	0	NULL	mAb 9C7	GP		bind					Hc proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_112_8_1164_s_299	14561701	( c) Binding of mAb 9C7 to  Hc proteins after serial treatment and reactivity of the  Hc-binding mAb s to recombinant protein (second through fourth lanes).	bind
2464	2	1510	5	10	NULL	0	NULL	Hc-binding mAbs	GP		reacts with					recombinant protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_112_8_1164_s_299	14561701	( c) Binding of mAb 9C7 to  Hc proteins after serial treatment and reactivity of the  Hc-binding mAb s to recombinant protein (second through fourth lanes).	bind
2465	3	1510	5	10	NULL	0	NULL	statement 1	Process		occurs after					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_112_8_1164_s_299	14561701	( c) Binding of mAb 9C7 to  Hc proteins after serial treatment and reactivity of the  Hc-binding mAb s to recombinant protein (second through fourth lanes).	bind
1747	1	1510	7	10	NULL	0	NULL	mAb 9C7	GP		bind					Hc proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_112_8_1164_s_299	14561701	( c) Binding of mAb 9C7 to  Hc proteins after serial treatment and reactivity of the  Hc-binding mAb s to recombinant protein (second through fourth lanes).	bind
1748	2	1510	7	10	NULL	0	NULL	Hc-binding mAbs	GP		reacts with					recombinant protein 	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_112_8_1164_s_299	14561701	( c) Binding of mAb 9C7 to  Hc proteins after serial treatment and reactivity of the  Hc-binding mAb s to recombinant protein (second through fourth lanes).	bind
1749	3	1510	7	10	NULL	0	NULL	statement 1	Process		occurs after					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_112_8_1164_s_299	14561701	( c) Binding of mAb 9C7 to  Hc proteins after serial treatment and reactivity of the  Hc-binding mAb s to recombinant protein (second through fourth lanes).	bind
1390	1	1511	5	10	NULL	0	NULL	NC	GP		bind					(TG)4	NucleicAcid			156.6 RU surface	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_2_472_s_114	16434700	( C) Binding of NC to a 156.6 RU surface of (TG)4.	bind
1750	1	1511	7	10	NULL	0	NULL	NC	GP		bind					(TG)4	NucleicAcid			156.6 RU surface of 	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_2_472_s_114	16434700	( C) Binding of NC to a 156.6 RU surface of (TG)4.	bind
1391	1	1512	5	10	NULL	0	NULL	ORCA1	GP		bind					Str	GP			RV fragment of the promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_18_16_4455_s_150	10449411	( C) Binding of ORCA1 to the RV fragment of the  Str promoter.	bind
1751	1	1512	7	10	NULL	0	NULL	ORCA1 	GP		bind					Str	GP			RV fragment in the promoter of 	NULL		NULL	NULL	NULL	NULL	gw60_embo_18_16_4455_s_150	10449411	( C) Binding of ORCA1 to the RV fragment of the  Str promoter.	bind
1392	1	1513	5	10	NULL	0	NULL	OspA	GP		bind					OspA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_106_4_561_s_75	10953031	( c) Binding of OspA with OspA.	bind
1752	1	1513	7	10	NULL	0	NULL	OspA	GP		bind					OspA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_106_4_561_s_75	10953031	( c) Binding of OspA with OspA.	bind
1393	1	1514	5	NULL	NULL	0	NULL	phyB	NULL		bind	NULL				PIF3	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_24_13419_s_88	11069292	( c) Binding of phyB and phyA to PIF3 as a function of phy input level.	bind
1394	2	1514	5	NULL	NULL	0	NULL	phyA	NULL		bind	NULL				PIF3	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_24_13419_s_88	11069292	( c) Binding of phyB and phyA to PIF3 as a function of phy input level.	bind
2467	3	1514	5	NULL	NULL	0	NULL	statement 1	NULL		is a function of	NULL				phy input level	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_24_13419_s_88	11069292	( c) Binding of phyB and phyA to PIF3 as a function of phy input level.	bind
2470	4	1514	5	NULL	NULL	0	NULL	statement 2	NULL		is a function of	NULL				phy input level	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_24_13419_s_88	11069292	( c) Binding of phyB and phyA to PIF3 as a function of phy input level.	bind
1753	3	1514	7	NULL	NULL	0	NULL	phyB	NULL		bind to	NULL				PIF3	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_24_13419_s_88	11069292	( c) Binding of phyB and phyA to PIF3 as a function of phy input level.	bind
1754	4	1514	7	NULL	NULL	0	NULL	phyA	NULL		bind to	NULL				PIF3	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_24_13419_s_88	11069292	( c) Binding of phyB and phyA to PIF3 as a function of phy input level.	bind
1755	5	1514	7	NULL	NULL	0	NULL	statement 3	NULL		is a function of 	NULL				phy input level	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_24_13419_s_88	11069292	( c) Binding of phyB and phyA to PIF3 as a function of phy input level.	bind
1756	6	1514	7	NULL	NULL	0	NULL	statement 4	NULL		is a function of 	NULL				phy input level	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_24_13419_s_88	11069292	( c) Binding of phyB and phyA to PIF3 as a function of phy input level.	bind
1395	1	1515	5	10	NULL	0	NULL	PriA Bs	GP		bind					ssiA strands	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_7_1593_s_164	11917020	( C) Binding of PriA Bs to  ssiA strands covered by SSB Bs.	bind
61155	2	1515	5	10	NULL	0	NULL	ssiA strands	NucleicAcid		covered by					SSB Bs	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_7_1593_s_164	11917020	( C) Binding of PriA Bs to  ssiA strands covered by SSB Bs.	bind
1757	1	1515	7	10	NULL	0	NULL	PriA Bs 	GP		bind					ssiA strands	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_7_1593_s_164	11917020	( C) Binding of PriA Bs to  ssiA strands covered by SSB Bs.	bind
61156	2	1515	7	10	NULL	0	NULL	ssiA strands	NucleicAcid		covered by					SSB Bs	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_7_1593_s_164	11917020	( C) Binding of PriA Bs to  ssiA strands covered by SSB Bs.	bind
1396	1	1516	5	10	NULL	0	NULL	CtBP	GP	recombinant	bind					GST-E1ACter	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_295_5561_1895_s_22	11847309	( C) Binding of recombinant CtBP to GST-E1A at various concentrations of NAD+ and NADH. Glutathione beads were coated with GST-E1ACter (COOH-terminal 67 amino acids of E1A), and bound CtBP was quantified by Western blotting.	bind
2729	2	1516	5	10	NULL	0	NULL	GST E1ACter	GP		is					COOH-terminal 67 amino acids of E1A	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_295_5561_1895_s_22	11847309	( C) Binding of recombinant CtBP to GST-E1A at various concentrations of NAD+ and NADH. Glutathione beads were coated with GST-E1ACter (COOH-terminal 67 amino acids of E1A), and bound CtBP was quantified by Western blotting.	bind
1805	2	1516	7	10	NULL	0	NULL	CtBP	GP	recombinant	bind					GST-E1ACter	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_295_5561_1895_s_22	11847309	( C) Binding of recombinant CtBP to GST-E1A at various concentrations of NAD+ and NADH. Glutathione beads were coated with GST-E1ACter (COOH-terminal 67 amino acids of E1A), and bound CtBP was quantified by Western blotting.	bind
3200	1	1516	7	10	NULL	0	NULL	GST-E1ACter	GP		is					COOH-terminal 67 amino acids of E1A	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_295_5561_1895_s_22	11847309	( C) Binding of recombinant CtBP to GST-E1A at various concentrations of NAD+ and NADH. Glutathione beads were coated with GST-E1ACter (COOH-terminal 67 amino acids of E1A), and bound CtBP was quantified by Western blotting.	bind
1397	1	1517	5	10	NULL	0	NULL	ezrin	GP	recombinant	bind					SS phagosomes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_2_199_s_273	10637224	( C) Binding of recombinant ezrin to SS phagosomes.	bind
1807	2	1517	7	10	NULL	0	NULL	ezrin	GP	recombinant	bind					SS phagosomes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_2_199_s_273	10637224	( C) Binding of recombinant ezrin to SS phagosomes.	bind
1400	1	1518	5	NULL	NULL	0	NULL	RPA-AB	NULL		bind	NULL				CPD/AA-10 duplex	NULL				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_16_4747_s_130	12907715	( C) Binding of RPA-AB to the CPD/AA-10 duplex as a function of DNA concentration in  the absence (upper) and presence (lower) of equimolar XPA-MBD.	bind
2475	2	1518	5	NULL	NULL	0	NULL	statement 1	NULL		is a function of	NULL				DNA concentration	NULL				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_31_16_4747_s_130	12907715	( C) Binding of RPA-AB to the CPD/AA-10 duplex as a function of DNA concentration in  the absence (upper) and presence (lower) of equimolar XPA-MBD.	bind
1808	3	1518	7	NULL	NULL	0	NULL	RPA-AB	NULL		bind to	NULL				 CPD/AA-10 duplex 	NULL				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_16_4747_s_130	12907715	( C) Binding of RPA-AB to the CPD/AA-10 duplex as a function of DNA concentration in  the absence (upper) and presence (lower) of equimolar XPA-MBD.	bind
1810	5	1518	7	NULL	NULL	0	NULL	statement 3	NULL		is a function of 	NULL				DNA concentration	NULL				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_16_4747_s_130	12907715	( C) Binding of RPA-AB to the CPD/AA-10 duplex as a function of DNA concentration in  the absence (upper) and presence (lower) of equimolar XPA-MBD.	bind
1402	1	1519	5	10	NULL	0	NULL	RPA-AB	GP		bind					CPD/AA-10 duplex	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_16_4747_s_130	12907715	( C) Binding of RPA-AB to the CPD/AA-10 duplex as a function of DNA concentration in the absence (upper) and presence (lower) of equimolar XPA-MBD.	bind
49374	2	1519	7	10	NULL	0	NULL	RPA-AB	GP		bind					CPD/AA-10 duplex	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_16_4747_s_130	12907715	( C) Binding of RPA-AB to the CPD/AA-10 duplex as a function of DNA concentration in the absence (upper) and presence (lower) of equimolar XPA-MBD.	bind
1403	1	1520	5	10	NULL	0	NULL	C2A-C2B	GP	soluble	bind					C2A-C2B	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_4_2082_s_100	12578982	( C) Binding of soluble C2A-C2B from syt I (3 muM) to immobilized C2A-C2B from syt II  was assayed as described in  B.	bind
1812	2	1520	7	10	NULL	0	NULL	C2A-C2B	GP	soluble	bind					C2A-C2B	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_4_2082_s_100	12578982	( C) Binding of soluble C2A-C2B from syt I (3 muM) to immobilized C2A-C2B from syt II  was assayed as described in  B.	bind
1404	1	1521	5	10	NULL	0	NULL	FGF-7	GP	soluble	bind					perlecan	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_8_1599_s_182	9788974	( C) Binding of soluble FGF-7 to immobilized perlecan or type I collagen as  detected by protein overlay assay and immunoblotting.	bind
1405	2	1521	5	10	NULL	0	NULL	FGF-7	GP	soluble	bind					type I collagen	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_8_1599_s_182	9788974	( C) Binding of soluble FGF-7 to immobilized perlecan or type I collagen as  detected by protein overlay assay and immunoblotting.	bind
1813	1	1521	7	10	NULL	0	NULL	FGF-7	GP	soluble	bind 					perlecan	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_8_1599_s_182	9788974	( C) Binding of soluble FGF-7 to immobilized perlecan or type I collagen as  detected by protein overlay assay and immunoblotting.	bind
1814	2	1521	7	10	NULL	0	NULL	FGF-7	GP	soluble	bind					type I collagen	GP	 immobilized 			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_8_1599_s_182	9788974	( C) Binding of soluble FGF-7 to immobilized perlecan or type I collagen as  detected by protein overlay assay and immunoblotting.	bind
1406	1	1522	5	NULL	NULL	0	NULL	Sp1	NULL		bind	NULL				Sp1	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_science_296_5576_2238_s_80	11988536	( C) Binding of Sp1 to the D2 promoter is inhibited in the caudate of the human HD postmortem brain.	bind
1407	2	1522	5	NULL	NULL	0	NULL	statement 1	NULL		inhibited in	NULL				human HD postmortem brain	NULL	caudate			NULL		NULL	NULL	NULL	NULL	gw60_science_296_5576_2238_s_80	11988536	( C) Binding of Sp1 to the D2 promoter is inhibited in the caudate of the human HD postmortem brain.	bind
1815	3	1522	7	NULL	NULL	0	NULL	Sp1	NULL		bind to	NULL				D2	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_science_296_5576_2238_s_80	11988536	( C) Binding of Sp1 to the D2 promoter is inhibited in the caudate of the human HD postmortem brain.	bind
1816	4	1522	7	NULL	NULL	0	NULL	statement 3	NULL		is inhibited 	NULL				human HD postmortem brain	NULL	in the caudate of  			NULL		NULL	NULL	NULL	NULL	gw60_science_296_5576_2238_s_80	11988536	( C) Binding of Sp1 to the D2 promoter is inhibited in the caudate of the human HD postmortem brain.	bind
1408	1	1523	5	10	NULL	0	NULL	Spc29p	GP		bind					Bbp1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_3_421_s_44	10654940	( C) Binding of Spc29p to Bbp1p.	bind
1817	1	1523	7	10	NULL	0	NULL	Spc29p	GP		bind					Bbp1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_3_421_s_44	10654940	( C) Binding of Spc29p to Bbp1p.	bind
1409	1	1524	5	NULL	NULL	0	NULL		NULL		bind	NULL		R domain fragments			NULL		GST-N-Tail		NULL		NULL	NULL	NULL	NULL	gw60_science_286_5439_544_s_101	10521352	( C) Binding of the indicated R domain fragments to GST-N-Tail (2.85 muM).	bind
1818	1	1524	7	10	NULL	0	NULL		NULL	 	bind	NULL		R domain fragments			NULL		GST-N-Tail		NULL		NULL	NULL	NULL	NULL	gw60_science_286_5439_544_s_101	10521352	( C) Binding of the indicated R domain fragments to GST-N-Tail (2.85 muM).	bind
1410	1	1525	5	10	NULL	0	NULL	Plk1	GP		bind			PBD		Cdc25C	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_science_299_5610_1228_s_89	12595692	( C) Binding of the Plk1 PBD to Cdc25C in vivo.	bind
1819	1	1525	7	10	NULL	0	NULL	Plk1 	GP		bind 			PBD		Cdc25C	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_science_299_5610_1228_s_89	12595692	( C) Binding of the Plk1 PBD to Cdc25C in vivo.	bind
1411	1	1526	5	10	NULL	0	NULL	SnoN fragments	GP		bind					Smad2	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5440_771_s_36	10531062	( C) Binding of the SnoN fragments to Smad2 and Smad4.	bind
1412	2	1526	5	10	NULL	0	NULL	SnoN fragments	GP		bind					Smad4	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5440_771_s_36	10531062	( C) Binding of the SnoN fragments to Smad2 and Smad4.	bind
1820	1	1526	7	10	NULL	0	NULL	SnoN fragments	GP		bind					Smad2	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5440_771_s_36	10531062	( C) Binding of the SnoN fragments to Smad2 and Smad4.	bind
1821	2	1526	7	10	NULL	0	NULL	SnoN fragments	GP		bind					Smad4	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5440_771_s_36	10531062	( C) Binding of the SnoN fragments to Smad2 and Smad4.	bind
1413	1	1527	5	10	NULL	0	NULL	TIF32	GP		bind					GST - HCR1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_20_4_891_s_59	11179233	( C) Binding of TIF32 and PRT1 to GST - HCR1  in vitro.	bind
1414	2	1527	5	10	NULL	0	NULL	PRT1	GP		bind					GST - HCR1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_20_4_891_s_59	11179233	( C) Binding of TIF32 and PRT1 to GST - HCR1  in vitro.	bind
1822	1	1527	7	10	NULL	0	NULL	TIF32	GP		bind					GST - HCR1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_20_4_891_s_59	11179233	( C) Binding of TIF32 and PRT1 to GST - HCR1  in vitro.	bind
1823	2	1527	7	10	NULL	0	NULL	PRT1	GP		bind					GST - HCR1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_20_4_891_s_59	11179233	( C) Binding of TIF32 and PRT1 to GST - HCR1  in vitro.	bind
1415	1	1528	5	10	NULL	0	NULL	p100	GP	transfected	bind					IKKalpha	GP	endogenous			NULL	Tax-expressing cells	NULL	NULL	NULL	NULL	gw60_embo_20_23_6805_s_190	11726516	( C) Binding of transfected p100 to endogenous IKKalpha in Tax-expressing cells.	bind
1824	1	1528	7	10	NULL	0	NULL	p100	GP	transfected 	bind 					IKKalpha	GP	endogenous			NULL	Tax-expressing cells	NULL	NULL	NULL	NULL	gw60_embo_20_23_6805_s_190	11726516	( C) Binding of transfected p100 to endogenous IKKalpha in Tax-expressing cells.	bind
1416	1	1529	5	10	NULL	0	NULL	trastuzumab Fc variants	GP		bind					FcgammaRIIb	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_11_4005_s_47	16537476	( C) Binding of trastuzumab Fc variants to human FcgammaRIIb ( n = 2).	bind
1825	1	1529	7	10	NULL	0	NULL	trastuzumab Fc variants	GP		bind					FcgammaRIIb	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_11_4005_s_47	16537476	( C) Binding of trastuzumab Fc variants to human FcgammaRIIb ( n = 2).	bind
1417	1	1530	5	10	NULL	0	NULL	Ub	GP		bind					Dsk2p	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_2_745_s_106	11805328	( C) Binding of Ub to Dsk2p.	bind
1826	1	1530	7	10	NULL	0	NULL	Ub	GP		bind					Dsk2p	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_2_745_s_106	11805328	( C) Binding of Ub to Dsk2p.	bind
1418	1	1531	5	NULL	NULL	0	NULL	Lt rREL1	NULL	unlabeled purified	bind	NULL				L-complex	NULL	REL1-depleted			NULL		0	NULL	NULL	NULL	gw70_pnas_102_13_4712_s_156	15781861	( C) Binding of unlabeled purified Lt rREL1 to REL1-depleted L-complex.	bind
1843	2	1531	7	NULL	NULL	0	NULL	Lt rREL1	NULL	unlabeled purified	bind to	NULL				 L-complex	NULL	REL1-depleted			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_13_4712_s_156	15781861	( C) Binding of unlabeled purified Lt rREL1 to REL1-depleted L-complex.	bind
1419	1	1532	5	10	NULL	0	NULL	UNR	GP		bind					ARS RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_236	16356927	( C) Binding of UNR to the ARS RNA.	bind
1844	1	1532	7	10	NULL	0	NULL	UNR	GP		bind					 ARS RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_236	16356927	( C) Binding of UNR to the ARS RNA.	bind
1420	1	1533	5	10	NULL	0	NULL	vezatin	GP		bind					myosin VIIA	GP		C-terminal FERM domain		NULL		NULL	NULL	NULL	NULL	gw60_embo_19_22_6020_s_66	11080149	( C) Binding of vezatin to the myosin VIIA C-terminal FERM domain.	bind
1845	1	1533	7	10	NULL	0	NULL	vezatin	GP		bind					myosin VIIA	GP		C-terminal FERM domain		NULL		NULL	NULL	NULL	NULL	gw60_embo_19_22_6020_s_66	11080149	( C) Binding of vezatin to the myosin VIIA C-terminal FERM domain.	bind
1421	1	1534	5	10	NULL	0	NULL	Penelope EN	GP	WT	bind					ps1 target	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_41_14719_s_148	15465912	( C) Binding of WT  Penelope EN to the ps1 target at different concentrations of poly(dI).	bind
1846	1	1534	7	10	NULL	0	NULL	Penelope EN	GP	WT	bind					ps1 target	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_41_14719_s_148	15465912	( C) Binding of WT  Penelope EN to the ps1 target at different concentrations of poly(dI).	bind
1422	1	1535	5	10	NULL	0	NULL	XDRP1	GP		bind					A-type cyclins	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5009_s_99	10487753	( C) Binding of XDRP1 to other A-type cyclins.	bind
1847	1	1535	7	10	NULL	0	NULL	XDRP1	GP		bind					A-type cyclins	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5009_s_99	10487753	( C) Binding of XDRP1 to other A-type cyclins.	bind
1423	1	1536	5	NULL	NULL	0	NULL	ZO-2	NULL		bind	NULL				Ad9	NULL			 E4-ORF1	NULL		NULL	NULL	NULL	NULL	gw60_embo_20_20_5578_s_70	11598001	( C) Binding of ZO-2 to Ad9 E4-ORF1 but not to Ad5 and Ad12 E4-ORF1 in GST pulldown assays.	bind
1424	2	1536	5	NULL	NULL	0	NULL	ZO-2	NULL		does not bind	NULL				Ad5	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_20_20_5578_s_70	11598001	( C) Binding of ZO-2 to Ad9 E4-ORF1 but not to Ad5 and Ad12 E4-ORF1 in GST pulldown assays.	bind
1425	3	1536	5	NULL	NULL	0	NULL	ZO-2	NULL		bind	NULL				Ad12	NULL			 E4-ORF1	NULL		NULL	NULL	NULL	NULL	gw60_embo_20_20_5578_s_70	11598001	( C) Binding of ZO-2 to Ad9 E4-ORF1 but not to Ad5 and Ad12 E4-ORF1 in GST pulldown assays.	bind
1848	4	1536	7	NULL	NULL	0	NULL	ZO-2	NULL		bind to	NULL				Ad9 	NULL			E4-ORF1	NULL		0	NULL	NULL	NULL	gw60_embo_20_20_5578_s_70	11598001	( C) Binding of ZO-2 to Ad9 E4-ORF1 but not to Ad5 and Ad12 E4-ORF1 in GST pulldown assays.	bind
1849	5	1536	7	NULL	NULL	0	NULL	ZO-2	NULL		does not bind	NULL				Ad5	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_20_20_5578_s_70	11598001	( C) Binding of ZO-2 to Ad9 E4-ORF1 but not to Ad5 and Ad12 E4-ORF1 in GST pulldown assays.	bind
1850	6	1536	7	NULL	NULL	0	NULL	ZO-2	NULL		does not bind	NULL				Ad12 	NULL			E4-ORF1	NULL		0	NULL	NULL	NULL	gw60_embo_20_20_5578_s_70	11598001	( C) Binding of ZO-2 to Ad9 E4-ORF1 but not to Ad5 and Ad12 E4-ORF1 in GST pulldown assays.	bind
1426	1	1537	5	10	NULL	0	NULL	TGF-beta2	GP		bind					TGF-beta receptors	GP				NULL	cell surface of Mv1Lu cells	NULL	NULL	NULL	NULL	gw60_embo_20_3_480_s_93	11157754	( C) Binding of [125]TGF-beta2 to TGF-beta receptors at the cell surface of Mv1Lu and R1b/L17 cells.	bind
49523	2	1537	5	10	NULL	0	NULL	TGF-beta2	GP		bind					TGF-beta receptor	GP				NULL	cell surface of R1b/L17 cells	NULL	NULL	NULL	NULL	gw60_embo_20_3_480_s_93	11157754	( C) Binding of [125]TGF-beta2 to TGF-beta receptors at the cell surface of Mv1Lu and R1b/L17 cells.	bind
1851	1	1537	7	10	NULL	0	NULL	TGF-beta2	GP		bind					TGF-beta receptors	GP				NULL	cell surface of Mv1Lu cells	NULL	NULL	NULL	NULL	gw60_embo_20_3_480_s_93	11157754	( C) Binding of [125]TGF-beta2 to TGF-beta receptors at the cell surface of Mv1Lu and R1b/L17 cells.	bind
49524	2	1537	7	10	NULL	0	NULL	TGF-beta2	GP		bind					TGF-beta receptor	GP				NULL	cell surface of R1b/L17 cells	NULL	NULL	NULL	NULL	gw60_embo_20_3_480_s_93	11157754	( C) Binding of [125]TGF-beta2 to TGF-beta receptors at the cell surface of Mv1Lu and R1b/L17 cells.	bind
1427	1	1538	5	NULL	NULL	0	NULL	platelet P-selectin	NULL		bind	NULL				PSGL-1	NULL	microparticle			NULL		0	NULL	NULL	NULL	gw70_jclininvest_115_12_3355_s_172	16322780	( C) Blood-borne tissue factor associated with microparticles accumulates on the platelet  thrombus through the binding of platelet P-selectin and microparticle PSGL-1.	bind
1428	2	1538	5	NULL	NULL	0	NULL	blood-borne tissue factor	NULL		associate with	NULL				microparticles	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_115_12_3355_s_172	16322780	( C) Blood-borne tissue factor associated with microparticles accumulates on the platelet  thrombus through the binding of platelet P-selectin and microparticle PSGL-1.	bind
2478	3	1538	5	NULL	NULL	0	NULL	statement 2	NULL		accumulates on	NULL				platelet thrombus	NULL				NULL		0	NULL	NULL	NULL	gw70_jclininvest_115_12_3355_s_172	16322780	( C) Blood-borne tissue factor associated with microparticles accumulates on the platelet  thrombus through the binding of platelet P-selectin and microparticle PSGL-1.	bind
2479	4	1538	5	NULL	NULL	0	NULL	statement 3	NULL		occurs through	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jclininvest_115_12_3355_s_172	16322780	( C) Blood-borne tissue factor associated with microparticles accumulates on the platelet  thrombus through the binding of platelet P-selectin and microparticle PSGL-1.	bind
1855	3	1538	7	NULL	NULL	0	NULL	P-selectin	NULL	platelet	bind to	NULL				PSGL-1	NULL	microparticle			NULL		0	NULL	NULL	NULL	gw70_jclininvest_115_12_3355_s_172	16322780	( C) Blood-borne tissue factor associated with microparticles accumulates on the platelet  thrombus through the binding of platelet P-selectin and microparticle PSGL-1.	bind
1856	4	1538	7	NULL	NULL	0	NULL	Blood-borne tissue factor	NULL		associate with	NULL				microparticles	NULL				NULL		0	NULL	NULL	NULL	gw70_jclininvest_115_12_3355_s_172	16322780	( C) Blood-borne tissue factor associated with microparticles accumulates on the platelet  thrombus through the binding of platelet P-selectin and microparticle PSGL-1.	bind
1857	5	1538	7	NULL	NULL	0	NULL	statement 4	NULL		accumulates on	NULL				platelet thrombus	NULL				NULL		0	NULL	NULL	NULL	gw70_jclininvest_115_12_3355_s_172	16322780	( C) Blood-borne tissue factor associated with microparticles accumulates on the platelet  thrombus through the binding of platelet P-selectin and microparticle PSGL-1.	bind
1858	6	1538	7	NULL	NULL	0	NULL	statement 5	NULL		occurs through	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_115_12_3355_s_172	16322780	( C) Blood-borne tissue factor associated with microparticles accumulates on the platelet  thrombus through the binding of platelet P-selectin and microparticle PSGL-1.	bind
1429	1	1539	5	10	NULL	0	NULL	Asf1	GP	full-length	interact with					RFC	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_11_1365_s_217	15901673	( C) Both full-length and the N terminus of Asf1 interact with RFC.	bind
1430	2	1539	5	10	NULL	0	NULL	Asf1	GP		interact with			N terminus		RFC	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_11_1365_s_217	15901673	( C) Both full-length and the N terminus of Asf1 interact with RFC.	bind
1853	1	1539	7	10	NULL	0	NULL	Asf1	GP	full-length	interact with					RFC	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_11_1365_s_217	15901673	( C) Both full-length and the N terminus of Asf1 interact with RFC.	bind
1854	2	1539	7	10	NULL	0	NULL	Asf1	GP		interact with			N terminus		RFC	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_11_1365_s_217	15901673	( C) Both full-length and the N terminus of Asf1 interact with RFC.	bind
506	1	1540	5	NULL	NULL	0	NULL	LIF	NULL		bind	NULL				gp130 receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_21_11563_s_181	11016970	( c) Both LIF and IL-6 bind to the gp130 receptor and initiate signal transduction through Janus kinase-signal transducers and activators of transcription (STAT) pathways.	bind
507	2	1540	5	NULL	NULL	0	NULL	IL-6	NULL		bind	NULL				gp130 receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_21_11563_s_181	11016970	( c) Both LIF and IL-6 bind to the gp130 receptor and initiate signal transduction through Janus kinase-signal transducers and activators of transcription (STAT) pathways.	bind
508	3	1540	5	NULL	NULL	0	NULL	statement 1	NULL		initiate	NULL				signal transduction	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11563_s_181	11016970	( c) Both LIF and IL-6 bind to the gp130 receptor and initiate signal transduction through Janus kinase-signal transducers and activators of transcription (STAT) pathways.	bind
509	4	1540	5	NULL	NULL	0	NULL	statement 2	NULL		initiate	NULL				signal transduction	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11563_s_181	11016970	( c) Both LIF and IL-6 bind to the gp130 receptor and initiate signal transduction through Janus kinase-signal transducers and activators of transcription (STAT) pathways.	bind
510	5	1540	5	NULL	NULL	0	NULL	statement 1	NULL		occurs through	NULL				Janus kinase-STAT pathway	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11563_s_181	11016970	( c) Both LIF and IL-6 bind to the gp130 receptor and initiate signal transduction through Janus kinase-signal transducers and activators of transcription (STAT) pathways.	bind
2491	6	1540	5	NULL	NULL	0	NULL	statement 2	NULL		occurs through	NULL				Janus kinase-STAT pathway	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_21_11563_s_181	11016970	( c) Both LIF and IL-6 bind to the gp130 receptor and initiate signal transduction through Janus kinase-signal transducers and activators of transcription (STAT) pathways.	bind
2494	7	1540	5	NULL	NULL	0	NULL	Janus kinase-STAT	NULL		is	NULL				Janus kinase-signal transducers and activators of transcription	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_21_11563_s_181	11016970	( c) Both LIF and IL-6 bind to the gp130 receptor and initiate signal transduction through Janus kinase-signal transducers and activators of transcription (STAT) pathways.	bind
1859	6	1540	7	NULL	NULL	0	NULL	LIF	NULL		bind to	NULL				gp130 receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_21_11563_s_181	11016970	( c) Both LIF and IL-6 bind to the gp130 receptor and initiate signal transduction through Janus kinase-signal transducers and activators of transcription (STAT) pathways.	bind
1860	7	1540	7	NULL	NULL	0	NULL	IL-6	NULL		bind to	NULL				gp130 receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_21_11563_s_181	11016970	( c) Both LIF and IL-6 bind to the gp130 receptor and initiate signal transduction through Janus kinase-signal transducers and activators of transcription (STAT) pathways.	bind
1861	8	1540	7	NULL	NULL	0	NULL	statement 6	NULL		initiate	NULL				signal transduction	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11563_s_181	11016970	( c) Both LIF and IL-6 bind to the gp130 receptor and initiate signal transduction through Janus kinase-signal transducers and activators of transcription (STAT) pathways.	bind
1862	9	1540	7	NULL	NULL	0	NULL	statement 7	NULL		initiate	NULL				 signal transduction 	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11563_s_181	11016970	( c) Both LIF and IL-6 bind to the gp130 receptor and initiate signal transduction through Janus kinase-signal transducers and activators of transcription (STAT) pathways.	bind
1863	10	1540	7	NULL	NULL	0	NULL	statement 8	NULL		occurs through	NULL				Janus kinase-STAT pathway	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11563_s_181	11016970	( c) Both LIF and IL-6 bind to the gp130 receptor and initiate signal transduction through Janus kinase-signal transducers and activators of transcription (STAT) pathways.	bind
1864	11	1540	7	NULL	NULL	0	NULL	statement 9	NULL		occurs through	NULL				Janus kinase-STAT pathway	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11563_s_181	11016970	( c) Both LIF and IL-6 bind to the gp130 receptor and initiate signal transduction through Janus kinase-signal transducers and activators of transcription (STAT) pathways.	bind
2209	12	1540	7	NULL	NULL	0	NULL	Janus kinase-STAT	NULL		is	NULL				Janus kinase-signal transducers and activators of transcription	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_21_11563_s_181	11016970	( c) Both LIF and IL-6 bind to the gp130 receptor and initiate signal transduction through Janus kinase-signal transducers and activators of transcription (STAT) pathways.	bind
2078	1	1541	6	10	NULL	0	NULL	noggin	GP		bind					BMP4	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_274_5290_1115_s_46	8895454	( C) Both noggin and chordin bind to BMP4.	bind
2079	2	1541	6	10	NULL	0	NULL	chordin	GP		bind					BMP4	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_274_5290_1115_s_46	8895454	( C) Both noggin and chordin bind to BMP4.	bind
2080	1	1542	6	10	NULL	0	NULL	C-Mad2	GP		bind					Mad1	GP			Mad2-binding site	NULL		NULL	NULL	NULL	NULL	gw70_embo_25_6_1273_s_51	16525508	( C) C-Mad2 bound to the Mad2-binding site of Mad1 (green, PDB ID 1GO4).	bind
2081	1	1543	6	10	NULL	0	NULL	CCT	GP		bind					Gbeta	GP	deletion mutants			NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_22_8360_s_93	16717193	( C) CCT binding to Gbeta deletion mutants.	bind
2088	1	1545	6	10	NULL	0	NULL	CDC20	GP	mutant	bind		less			Mad2	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_279_5353_1041_s_93	9461437	( C) Checkpoint-resistant  CDC20 mutants have diminished binding of Mad2 and Mad3.	bind
2089	2	1545	6	10	NULL	0	NULL	CDC20	GP	mutant	bind		less			Mad3	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_279_5353_1041_s_93	9461437	( C) Checkpoint-resistant  CDC20 mutants have diminished binding of Mad2 and Mad3.	bind
2090	1	1547	6	10	NULL	0	NULL	PPARgamma	GP		associate with					GyK gene	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_4_453_s_76	15681609	( C) ChIP analysis of PPARgamma association with GyK and aP2 genes.	bind
2091	2	1547	6	10	NULL	0	NULL	PPARgamma	GP		associate with					aP2 gene	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_4_453_s_76	15681609	( C) ChIP analysis of PPARgamma association with GyK and aP2 genes.	bind
2092	1	1548	6	10	NULL	0	NULL	Myc proteins	GP		bind					hTERT	GP	exogenous		promoter	NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_14_8211_s_176	12821782	( C) CHIP assay  detects Myc and high-risk E6 proteins bound to an exogenous hTERT promoter.	bind
2093	2	1548	6	10	NULL	0	NULL	E6 proteins	GP	high-risk	bind					hTERT	GP	exogenous		promoter	NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_14_8211_s_176	12821782	( C) CHIP assay  detects Myc and high-risk E6 proteins bound to an exogenous hTERT promoter.	bind
2094	1	1549	6	10	NULL	0	NULL	HDAC1	GP		bind					HMG-CoA synthase	GP	endogenous;;mitochondrial		promoter	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_6_1693_s_144	12626711	( C) ChIP assay of HDAC1 bound to endogenous mitochondrial HMG-CoA synthase promoter.	bind
2095	1	1550	6	10	NULL	0	NULL	Nkx6.1	GP		bind					glucagon	GP	endogenous		promoter	NULL	class 3 cell line (832/3)	NULL	NULL	NULL	NULL	gw70_pnas_102_20_7297_s_150	15883383	( C) ChIP assay of Nkx6.1 binding to the endogenous glucagon promoter in a class 3 cell  line (832/3).	bind
2096	1	1551	6	10	NULL	0	NULL	RUNX1	GP		bind		specifically			MIP-1alpha	GP	endogenous		promoter	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_11_2735_s_129	12771199	( C) ChIP assays demonstrating specific binding of RUNX1 to the endogenous MIP-1alpha promoter.	bind
2097	1	1552	6	10	NULL	0	NULL	Dnmt3a	GP		does not bind					ODC	GP				NULL	c-myc+/+ cells	NULL	NULL	NULL	NULL	gw70_embo_24_2_336_s_134	15616584	( C) ChIPs performed in  c-myc+/+ cells show that Dnmt3a does not bind the Myc-activated E-box genes  ODC and  NM23-H2.	bind
2098	2	1552	6	10	NULL	0	NULL	Dnmt3a	GP		does not bind					NM23-H2	GP				NULL	c-myc+/+ cells	NULL	NULL	NULL	NULL	gw70_embo_24_2_336_s_134	15616584	( C) ChIPs performed in  c-myc+/+ cells show that Dnmt3a does not bind the Myc-activated E-box genes  ODC and  NM23-H2.	bind
46172	3	1552	6	10	NULL	0	NULL	Myc	GP		activates					E-box genes	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_2_336_s_134	15616584	( C) ChIPs performed in  c-myc+/+ cells show that Dnmt3a does not bind the Myc-activated E-box genes  ODC and  NM23-H2.	bind
46173	4	1552	6	10	NULL	0	NULL	ODC	GP		is a type of					E-box genes	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_2_336_s_134	15616584	( C) ChIPs performed in  c-myc+/+ cells show that Dnmt3a does not bind the Myc-activated E-box genes  ODC and  NM23-H2.	bind
46174	5	1552	6	10	NULL	0	NULL	NM23-H2	GP		is a type of					E-box genes	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_2_336_s_134	15616584	( C) ChIPs performed in  c-myc+/+ cells show that Dnmt3a does not bind the Myc-activated E-box genes  ODC and  NM23-H2.	bind
2099	1	1553	6	10	NULL	0	NULL	HMG-D	GP		bind					66 bp DNA circles	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_11_2852_s_193	12771212	( C) Circularization curves for L9, A36, V32 and T33 series of mutants and Spec. ( D) EMSA of HMG-D bound to the 66 bp DNA circles (lanes 1 - 8) and 77 bp circles (lanes  9 - 16).	bind
2100	2	1553	6	10	NULL	0	NULL	HMG-D	GP		bind					77 bp DNA circles	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_11_2852_s_193	12771212	( C) Circularization curves for L9, A36, V32 and T33 series of mutants and Spec. ( D) EMSA of HMG-D bound to the 66 bp DNA circles (lanes 1 - 8) and 77 bp circles (lanes  9 - 16).	bind
2190	1	1556	6	10	NULL	0	NULL	HEXIM1	GP		oligomerizes in					cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7000_s_155	16377779	( C) Combined disruptions of the CR and the 7SK snRNA binding site abolish completely  HEXIM1 oligomerization in cells.	bind
2191	2	1556	6	10	NULL	0	NULL			disruption of	abolish		completely	 CR 		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7000_s_155	16377779	( C) Combined disruptions of the CR and the 7SK snRNA binding site abolish completely  HEXIM1 oligomerization in cells.	bind
52600	3	1556	6	10	NULL	0	NULL			disruption of	abolish		completely	7SK snRNA binding site		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7000_s_155	16377779	( C) Combined disruptions of the CR and the 7SK snRNA binding site abolish completely  HEXIM1 oligomerization in cells.	bind
2101	1	1557	6	10	NULL	0	NULL	TFIIB	GP		bind					Xist P1	GP			promoter	NULL	female TS cells	NULL	NULL	NULL	NULL	gw70_genesdev_19_12_1474_s_139	15964997	( C) Comparative analysis of the  Xist/Tsix transcripts ratio (black bars) with the ratio of TFIIB binding to  Xist P1 promoter versus  Tsix promoter (gray bars) in female TS cells, ES cells, and MEFs.	bind
2102	2	1557	6	10	NULL	0	NULL	TFIIB	GP		bind					Tsix 	GP			promoter	NULL	female TS cells	NULL	NULL	NULL	NULL	gw70_genesdev_19_12_1474_s_139	15964997	( C) Comparative analysis of the  Xist/Tsix transcripts ratio (black bars) with the ratio of TFIIB binding to  Xist P1 promoter versus  Tsix promoter (gray bars) in female TS cells, ES cells, and MEFs.	bind
2103	3	1557	6	10	NULL	0	NULL	TFIIB	GP		bind					Xist P1	GP			promoter	NULL	ES cells	NULL	NULL	NULL	NULL	gw70_genesdev_19_12_1474_s_139	15964997	( C) Comparative analysis of the  Xist/Tsix transcripts ratio (black bars) with the ratio of TFIIB binding to  Xist P1 promoter versus  Tsix promoter (gray bars) in female TS cells, ES cells, and MEFs.	bind
2104	4	1557	6	10	NULL	0	NULL	TFIIB	GP		bind					Tsix 	GP			promoter	NULL	ES cells	NULL	NULL	NULL	NULL	gw70_genesdev_19_12_1474_s_139	15964997	( C) Comparative analysis of the  Xist/Tsix transcripts ratio (black bars) with the ratio of TFIIB binding to  Xist P1 promoter versus  Tsix promoter (gray bars) in female TS cells, ES cells, and MEFs.	bind
2105	5	1557	6	10	NULL	0	NULL	TFIIB	GP		bind					Xist P1	GP			promoter	NULL	MEFs	NULL	NULL	NULL	NULL	gw70_genesdev_19_12_1474_s_139	15964997	( C) Comparative analysis of the  Xist/Tsix transcripts ratio (black bars) with the ratio of TFIIB binding to  Xist P1 promoter versus  Tsix promoter (gray bars) in female TS cells, ES cells, and MEFs.	bind
2106	6	1557	6	10	NULL	0	NULL	TFIIB	GP		bind					Tsix 	GP			promoter	NULL	MEFs	NULL	NULL	NULL	NULL	gw70_genesdev_19_12_1474_s_139	15964997	( C) Comparative analysis of the  Xist/Tsix transcripts ratio (black bars) with the ratio of TFIIB binding to  Xist P1 promoter versus  Tsix promoter (gray bars) in female TS cells, ES cells, and MEFs.	bind
2107	1	1558	6	10	NULL	0	NULL	SRF	GP		bind					CFTR	GP			CArG box	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_16_5271_s_409	16170155	( C) Comparative binding of SRF to  CFTR CArG boxes.	bind
2108	1	1559	6	10	NULL	0	NULL	KaiA	GP	wild type	bind					KaiC	GP	His-tagged			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_8_1688_s_168	15071498	( C) Comparison of binding profiles of mutant and wild-type KaiA and KaiB proteins to  6x-His-tagged KaiC bound to Ni beads.	bind
2109	2	1559	6	10	NULL	0	NULL	KaiA	GP	mutant	bind					KaiC	GP	His-tagged			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_8_1688_s_168	15071498	( C) Comparison of binding profiles of mutant and wild-type KaiA and KaiB proteins to  6x-His-tagged KaiC bound to Ni beads.	bind
2110	3	1559	6	10	NULL	0	NULL	KaiB	GP	wild type	bind					KaiC	GP	His-tagged			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_8_1688_s_168	15071498	( C) Comparison of binding profiles of mutant and wild-type KaiA and KaiB proteins to  6x-His-tagged KaiC bound to Ni beads.	bind
2111	4	1559	6	10	NULL	0	NULL	KaiB	GP	mutant	bind					KaiC	GP	His-tagged			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_8_1688_s_168	15071498	( C) Comparison of binding profiles of mutant and wild-type KaiA and KaiB proteins to  6x-His-tagged KaiC bound to Ni beads.	bind
2112	1	1560	6	10	NULL	0	NULL	CFTR	GP		bind					GST-alpha1-AMPK 	GP		NH2-terminal		NULL	CHO-BQ2 cells	NULL	NULL	NULL	NULL	gw60_jclininvest_105_12_1711_s_149	10862786	( c) Comparison of binding strengths of CFTR with NH2-terminal and COOH-terminal GST-alpha1-AMPK fusion proteins in CHO-BQ2 cells.	bind
2113	2	1560	6	10	NULL	0	NULL	CFTR	GP		bind					GST-alpha1-AMPK 	GP		COOH-terminal		NULL	CHO-BQ2 cells	NULL	NULL	NULL	NULL	gw60_jclininvest_105_12_1711_s_149	10862786	( c) Comparison of binding strengths of CFTR with NH2-terminal and COOH-terminal GST-alpha1-AMPK fusion proteins in CHO-BQ2 cells.	bind
52601	3	1560	6	10	NULL	0	NULL	GST-alpha1-AMPK 	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_105_12_1711_s_149	10862786	( c) Comparison of binding strengths of CFTR with NH2-terminal and COOH-terminal GST-alpha1-AMPK fusion proteins in CHO-BQ2 cells.	bind
2114	1	1561	6	10	NULL	0	NULL	ICAM-2 peptide	GP		bind					radixin	GP		FERM domain		NULL		NULL	NULL	NULL	NULL	gw60_embo_22_3_502_s_213	12554651	( C) Comparison of the 310 helix in the ICAM-2 peptide bound to the radixin FERM domain with the beta-turn of the NPxY motif in the IR peptide bound to the IRS-1 PTB domain.	bind
2115	2	1561	6	10	NULL	0	NULL	IR peptide	GP		bind			beta-turn of the NPxY motif		IRS-1	GP		PTB domain		NULL		NULL	NULL	NULL	NULL	gw60_embo_22_3_502_s_213	12554651	( C) Comparison of the 310 helix in the ICAM-2 peptide bound to the radixin FERM domain with the beta-turn of the NPxY motif in the IR peptide bound to the IRS-1 PTB domain.	bind
2116	1	1562	6	10	NULL	0	NULL	m7G	Chemical		bind					CBP20	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_20_5548_s_115	12374755	( C) Comparison of the mode of m7G binding to CBP20, VP39 and eIF4E.	bind
2117	2	1562	6	10	NULL	0	NULL	m7G	Chemical		bind					VP39	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_20_5548_s_115	12374755	( C) Comparison of the mode of m7G binding to CBP20, VP39 and eIF4E.	bind
2118	3	1562	6	10	NULL	0	NULL	m7G	Chemical		bind					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_20_5548_s_115	12374755	( C) Comparison of the mode of m7G binding to CBP20, VP39 and eIF4E.	bind
2119	1	1563	6	10	NULL	0	NULL	QacR	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_5_1210_s_70	11867549	( C) Comparison of two TetR family members bound to DNA: QacR and TetR ( Orth  et al., 2000).	bind
2120	2	1563	6	10	NULL	0	NULL	TetR	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_5_1210_s_70	11867549	( C) Comparison of two TetR family members bound to DNA: QacR and TetR ( Orth  et al., 2000).	bind
2121	1	1564	6	10	NULL	0	NULL	SmpB	GP		bind					SsrA	GP	32P -labeled			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_13_3793_s_104	10393194	( C) Competition for binding of SmpB to 100 pM 32P -labeled SsrA by unlabeled SsrA RNA or total yeast tRNA.	bind
2122	2	1564	6	10	NULL	0	NULL	SmpB 	GP		bind					SsrA RNA	NucleicAcid	unlabeled			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_13_3793_s_104	10393194	( C) Competition for binding of SmpB to 100 pM 32P -labeled SsrA by unlabeled SsrA RNA or total yeast tRNA.	bind
2466	3	1564	6	10	NULL	0	NULL	statement 2	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_13_3793_s_104	10393194	( C) Competition for binding of SmpB to 100 pM 32P -labeled SsrA by unlabeled SsrA RNA or total yeast tRNA.	bind
2468	4	1564	6	10	NULL	0	NULL	total yeast tRNA	NucleicAcid	unlabeled	bind					SsrA	NucleicAcid	32P-labeled			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_13_3793_s_104	10393194	( C) Competition for binding of SmpB to 100 pM 32P -labeled SsrA by unlabeled SsrA RNA or total yeast tRNA.	bind
2469	5	1564	6	10	NULL	0	NULL	statement 4	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_13_3793_s_104	10393194	( C) Competition for binding of SmpB to 100 pM 32P -labeled SsrA by unlabeled SsrA RNA or total yeast tRNA.	bind
2124	1	1565	6	10	NULL	0	NULL	Ets1	GP		bind					28 bp oligonucleotide	GP			Ets-binding site 	NULL		NULL	NULL	NULL	NULL	gw60_embo_21_3_365_s_144	11823429	( C) Competition gel mobility shift assay for Ets1 binding to a 28 bp oligonucleotide (see Materials and methods) carrying an Ets-binding site.	bind
2125	1	1566	6	10	NULL	0	NULL	CRP	GP		bind					PC-KLH	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_20_13043_s_110	12244213	( C) Competition immunoassays for binding of CRP to PC-KLH.	bind
2126	1	1568	6	10	NULL	0	NULL	Stat2	GP		bind					p300	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_11_3124_s_45	9606194	( C) Competitive binding of Stat2 and RelA to p300 (CH1).	bind
2127	2	1568	6	10	NULL	0	NULL	RelA	GP		bind					p300	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_11_3124_s_45	9606194	( C) Competitive binding of Stat2 and RelA to p300 (CH1).	bind
2413	3	1568	6	10	NULL	0	NULL	statement 1	Process		compete with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_11_3124_s_45	9606194	( C) Competitive binding of Stat2 and RelA to p300 (CH1).	bind
2128	1	1569	6	10	NULL	0	NULL	IAA	Chemical		bind					insulin	GP	human	Tyr14A		NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_4_589_s_135	15314696	( C) Competitive inhibition of IAA binding to Tyr14A [125] human insulin using human proinsulin (filled circles) for each of the sera shown  in  B.	bind
2129	2	1569	6	10	NULL	0	NULL	proinsulin	GP	human	bind					IAA	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_4_589_s_135	15314696	( C) Competitive inhibition of IAA binding to Tyr14A [125] human insulin using human proinsulin (filled circles) for each of the sera shown  in  B.	bind
46175	3	1569	6	10	NULL	0	NULL	statement 1	Process		competes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_4_589_s_135	15314696	( C) Competitive inhibition of IAA binding to Tyr14A [125] human insulin using human proinsulin (filled circles) for each of the sera shown  in  B.	bind
2130	1	1571	6	10	NULL	0	NULL	malonyl-CoA	Chemical		bind					CPT1c	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_19_7282_s_55	16651524	( C) Concentration dependence of malonyl-CoA binding to CPT1c.	bind
2131	1	1573	6	10	NULL	0	NULL	spastin	GP		bind					atlastin	GP		C-tail		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_28_10666_s_46	16815977	( C) Coomassie blue-stained gel showing that spastin binds to the atlastin C-tail.	bind
2132	1	1574	6	10	NULL	0	NULL	DSX	GP		bind			DM domain		DNA	NucleicAcid			palindromic site 5''-ACTACA ATTGTTGCA-3''	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_14_1750_s_149	10898790	( C) Cooperative low-affinity binding of the DSX DM domain to a palindromic (sym) DNA site (5''-ACTACA ATTGTTGCA-3''; central base pair in boldface type) using fluorescein (at 5' of top strand) as probe.	bind
2133	1	1575	6	10	NULL	0	NULL	C3G	GP		bind					Trk	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_12_2358_s_164	15167895	( C) CrkL increases the binding of C3G and Trk upon NGF treatment.	bind
2134	3	1575	6	10	NULL	0	NULL	CrkL	GP		increases					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_12_2358_s_164	15167895	( C) CrkL increases the binding of C3G and Trk upon NGF treatment.	bind
2205	2	1575	6	10	NULL	0	NULL	NGF	GP		is required for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_12_2358_s_164	15167895	( C) CrkL increases the binding of C3G and Trk upon NGF treatment.	bind
2135	1	1576	6	10	NULL	0	NULL	eIF4E	GP	human	bind					m7GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_21_5138_s_113	17036047	( C) Crystal structure of human eIF4E bound to m7GDP (PDB 1EJ1).	bind
2136	1	1577	6	10	NULL	0	NULL	CID derivatives	GP		bind								CTD		NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_13_1572_s_138	15998810	( C) CTD pull-down analysis for binding between CID derivatives and the CTD.	bind
2137	1	1578	6	10	NULL	0	NULL	D-Axin	GP		bind					Arm	GP		Armadillo repeat domain		NULL		NULL	NULL	NULL	NULL	gw60_science_283_5408_1739_s_43	10073940	( C) D-Axin binds to the Armadillo repeat domain of Arm.	bind
2138	1	1580	6	10	NULL	0	NULL	LPS	Chemical		induces					IkappaBalpha	GP	degradation of 			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_7_873_s_61	12654725	( C) Degradation of IkappaBalpha induced by lipopolysaccharide (LPS) and interleukin-1beta (IL-1beta).	bind
2139	2	1580	6	10	NULL	0	NULL	IL-1beta	GP		induces					IkappaBalpha	GP	degradation of 			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_7_873_s_61	12654725	( C) Degradation of IkappaBalpha induced by lipopolysaccharide (LPS) and interleukin-1beta (IL-1beta).	bind
45914	3	1580	6	10	NULL	0	NULL	LPS	Chemical		is					lipopolysaccharide 	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_7_873_s_61	12654725	( C) Degradation of IkappaBalpha induced by lipopolysaccharide (LPS) and interleukin-1beta (IL-1beta).	bind
45916	4	1580	6	10	NULL	0	NULL	IL-1beta	GP		is					 interleukin-1beta	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_7_873_s_61	12654725	( C) Degradation of IkappaBalpha induced by lipopolysaccharide (LPS) and interleukin-1beta (IL-1beta).	bind
2140	1	1581	6	10	NULL	0	NULL	bradykinin	GP		bind					OppA	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_23_12487_s_79	11050157	( C) Determination of the dissociation constant ( Kd) for bradykinin binding to OppA.	bind
2141	1	1582	6	10	NULL	0	NULL	dFOXO	GP		bind		specifically			d4EBP	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_genesdev_17_16_2006_s_182	12893776	( C) dFOXO  binds specifically to d4EBP and dInR promoters in vivo.	bind
2142	2	1582	6	10	NULL	0	NULL	dFOXO	GP		bind		specifically			dInR	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_genesdev_17_16_2006_s_182	12893776	( C) dFOXO  binds specifically to d4EBP and dInR promoters in vivo.	bind
2143	1	1583	6	10	NULL	0	NULL	dFOXO	GP		bind					dInR	GP			promoter	NULL	S2 cells	NULL	NULL	NULL	NULL	gw70_genesdev_19_20_2435_s_71	16230533	( C) dFOXO binds to the dInR promoter in S2 cells upon starvation.	bind
52602	2	1583	6	10	NULL	0	NULL	statement 1	Process		occurs upon					starvation	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_20_2435_s_71	16230533	( C) dFOXO binds to the dInR promoter in S2 cells upon starvation.	bind
2144	1	1584	6	10	NULL	0	NULL	Rad18	GP		bind		directly			pol	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_19_3886_s_174	15359278	( C) Direct binding of Rad18 with pol .	bind
2145	1	1585	6	10	NULL	0	NULL				bind		directly	alphaX I domain					Glu		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1614_s_175	15665082	( C) Direct binding of the alphaX I domain to Glu.	bind
2146	1	1586	6	10	NULL	0	NULL	MBD1	GP		bind		directly	TRD		MPG	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_100_22_12859_s_73	14555760	( C) Direct binding of the TRD of MBD1 to MPG  in vitro.	bind
2147	1	1587	6	10	NULL	0	NULL	fibrillin	GP		bind					ABI2	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_15_6061_s_58	16571665	( C) Discriminative binding of fibrillin to ABI2 and mutant abi2 analyzed by pulldown  assay.	bind
2148	2	1587	6	10	NULL	0	NULL	fibrillin	GP		bind					abi2	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_15_6061_s_58	16571665	( C) Discriminative binding of fibrillin to ABI2 and mutant abi2 analyzed by pulldown  assay.	bind
2149	1	1589	6	10	NULL	0	NULL	DM	GP		counteracts					MBP peptides	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_6_1241_s_32	10716924	( C) DM counteracts binding of MBP peptides.	bind
2150	1	1590	6	10	NULL	0	NULL	R2 proteins	GP		bind					28S rRNA gene	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_20_6461_s_89	16284201	( C) DNA sequence of the 28S rRNA gene region bound by R2 proteins.	bind
2151	1	1591	6	10	NULL	0	NULL	NFAT5	GP		bind		competitively			ATF-2/c-jun	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_12_3845_s_154	16027109	( C) DNase I footprinting assay of competitive binding of NFAT5 and ATF-2/c-jun.	bind
203	1	1592	5	10	NULL	0	NULL	LEF1	GP	recombinant	bind							predicted		LEF/TCF site 	NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_9_6064_s_142	11983900	( C) DNase I footprinting revealing binding of recombinant LEF1 protein to the predicted LEF/TCF site (shown in bold).	bind
2152	1	1592	6	10	NULL	0	NULL	LEF1 protein	GP	recombinant	bind									LEF/TCF site	NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_9_6064_s_142	11983900	( C) DNase I footprinting revealing binding of recombinant LEF1 protein to the predicted LEF/TCF site (shown in bold).	bind
208	1	1593	5	10	NULL	0	NULL	Dnmt3L	GP		bind					HDAC1	GP	specific regions			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_17_3831_s_45	12202768	( C) Dnmt3L binds specific regions of HDAC1  in vitro.	bind
2153	1	1593	6	10	NULL	0	NULL	Dnmt3L	GP		bind					HDAC1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_17_3831_s_45	12202768	( C) Dnmt3L binds specific regions of HDAC1  in vitro.	bind
209	1	1594	5	10	NULL	0	NULL	griseofulvin	GP		bind					tubulin	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_28_9878_s_154	15985553	( C) Double-reciprocal plot for the binding of griseofulvin to tubulin.	bind
2154	2	1594	6	10	NULL	0	NULL	griseofulvin	GP		bind					tubulin	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_28_9878_s_154	15985553	( C) Double-reciprocal plot for the binding of griseofulvin to tubulin.	bind
210	1	1595	5	10	NULL	0	NULL	DRIP130	GP		bind		specifically			ESX	GP		activation domain		NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_20_12747_s_70	12242338	( C) DRIP130 binds specifically to the ESX activation domain.	bind
2155	1	1595	6	10	NULL	0	NULL	DRIP130	GP		bind		specifically			ESX	GP		activation domain		NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_20_12747_s_70	12242338	( C) DRIP130 binds specifically to the ESX activation domain.	bind
211	1	1596	5	10	NULL	0	NULL	c-Fos	GP		bind					TNF 	GP	probe		TRE site in promoter	NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_104_4_503_s_217	10449442	( c) E2 decreases the binding of c-Fos to a probe containing an exact copy of the TRE site in the TNF promoter.	bind
212	2	1596	5	10	NULL	0	NULL	E2	GP		decreases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_104_4_503_s_217	10449442	( c) E2 decreases the binding of c-Fos to a probe containing an exact copy of the TRE site in the TNF promoter.	bind
2156	3	1596	6	10	NULL	0	NULL	c-fos	GP		bind					TNF	GP			TRE site in promoter	NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_104_4_503_s_217	10449442	( c) E2 decreases the binding of c-Fos to a probe containing an exact copy of the TRE site in the TNF promoter.	bind
2157	4	1596	6	10	NULL	0	NULL	E2	GP		decreases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_104_4_503_s_217	10449442	( c) E2 decreases the binding of c-Fos to a probe containing an exact copy of the TRE site in the TNF promoter.	bind
222	1	1597	5	10	NULL	0	NULL	p35srj	GP		bind					p300	GP		CH1		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_genesdev_13_1_64_s_104	9887100	( C) Effect of p35srj 224-255 peptide on in vitro binding of p35srj to p300-CH1.	bind
2233	1	1597	6	10	NULL	0	NULL	p35srj	GP		bind					p300	GP		CH1		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_genesdev_13_1_64_s_104	9887100	( C) Effect of p35srj 224-255 peptide on in vitro binding of p35srj to p300-CH1.	bind
224	1	1598	5	10	NULL	0	NULL	La protein	GP		bind					BiP	GP			IRES	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_5009_s_130	11812831	( C) Effect of the initiator AUG on binding of La protein to the BiP IRES.	bind
2234	1	1598	6	10	NULL	0	NULL	La protein	GP		bind					BiP	GP			IRES	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_5009_s_130	11812831	( C) Effect of the initiator AUG on binding of La protein to the BiP IRES.	bind
226	1	1599	5	10	NULL	0	NULL	PSF protein	GP		bind					GAGE6	GP			promoter DNA	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_34_12189_s_105	16079199	( C) Effect of VL30 RNA on binding of PSF protein and DBD to  GAGE6 promoter DNA.	bind
227	2	1599	5	10	NULL	0	NULL				bind			DBD		GAGE6	GP			promoter DNA	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_34_12189_s_105	16079199	( C) Effect of VL30 RNA on binding of PSF protein and DBD to  GAGE6 promoter DNA.	bind
2235	1	1599	6	10	NULL	0	NULL	PSF protein	GP		bind					GAGE6	GP			promoter DNA	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_34_12189_s_105	16079199	( C) Effect of VL30 RNA on binding of PSF protein and DBD to  GAGE6 promoter DNA.	bind
2236	2	1599	6	10	NULL	0	NULL				bind			DBD		GAGE6	GP			promoter DNA	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_34_12189_s_105	16079199	( C) Effect of VL30 RNA on binding of PSF protein and DBD to  GAGE6 promoter DNA.	bind
272	1	1600	5	10	NULL	0	NULL	eIF4E	GP		bind					4E-T	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_12_3142_s_71	10856257	( C) eIF4E binds to 4E-T and eIF4G through a shared sequence.	bind
273	2	1600	5	10	NULL	0	NULL	eIF4E	GP		bind					eIF4G	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_12_3142_s_71	10856257	( C) eIF4E binds to 4E-T and eIF4G through a shared sequence.	bind
2237	1	1600	6	10	NULL	0	NULL	eIF4E	GP		bind					4E-T	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_12_3142_s_71	10856257	( C) eIF4E binds to 4E-T and eIF4G through a shared sequence.	bind
2238	2	1600	6	10	NULL	0	NULL	eIF4E	GP		bind					eIF4G	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_12_3142_s_71	10856257	( C) eIF4E binds to 4E-T and eIF4G through a shared sequence.	bind
274	1	1601	5	10	NULL	0	NULL	IgA	GP	intestinal secretory	bind					Xa-CAT 	GP	purified			NULL	wild-type E. coli expressing Xa-CAT  in the intestine in vivo	NULL	NULL	NULL	NULL	gw60_science_288_5474_2222_s_78	10864873	( C) ELISA of intestinal  secretory IgA or serum IgA binding to purified Xa-CAT chimeric protein  35 days after colonization with wild-type  E. coli expressing  this protein in the intestine in vivo.	bind
275	2	1601	5	10	NULL	0	NULL	IgA	GP	serum	bind					Xa-CAT	GP	purified			NULL	wild-type E. coli expressing Xa-CAT  in the intestine in vivo	NULL	NULL	NULL	NULL	gw60_science_288_5474_2222_s_78	10864873	( C) ELISA of intestinal  secretory IgA or serum IgA binding to purified Xa-CAT chimeric protein  35 days after colonization with wild-type  E. coli expressing  this protein in the intestine in vivo.	bind
46153	3	1601	5	10	NULL	0	NULL	Xa-CAT	GP		is a type of					chimeric protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_288_5474_2222_s_78	10864873	( C) ELISA of intestinal  secretory IgA or serum IgA binding to purified Xa-CAT chimeric protein  35 days after colonization with wild-type  E. coli expressing  this protein in the intestine in vivo.	bind
2239	1	1601	6	10	NULL	0	NULL	IgA	GP	intestinal secretory	bind					Xa-CAT 	GP	purified			NULL	wild-type E. coli expressing  Xa-CAT in the intestine in vivo	NULL	NULL	NULL	NULL	gw60_science_288_5474_2222_s_78	10864873	( C) ELISA of intestinal  secretory IgA or serum IgA binding to purified Xa-CAT chimeric protein  35 days after colonization with wild-type  E. coli expressing  this protein in the intestine in vivo.	bind
2240	2	1601	6	10	NULL	0	NULL	IgA	GP	serum	bind					Xa-CAT	GP	purified			NULL	wild-type E. coli expressing Xa-CAT in the intestine in vivo	NULL	NULL	NULL	NULL	gw60_science_288_5474_2222_s_78	10864873	( C) ELISA of intestinal  secretory IgA or serum IgA binding to purified Xa-CAT chimeric protein  35 days after colonization with wild-type  E. coli expressing  this protein in the intestine in vivo.	bind
46176	3	1601	6	10	NULL	0	NULL	Xa-CAT	GP		is a type of					chimeric protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_288_5474_2222_s_78	10864873	( C) ELISA of intestinal  secretory IgA or serum IgA binding to purified Xa-CAT chimeric protein  35 days after colonization with wild-type  E. coli expressing  this protein in the intestine in vivo.	bind
276	1	1602	5	10	NULL	0	NULL	p19ARF	GP	endogenous	bind					E2F1	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_8_4455_s_151	11274364	( C) Endogenous p19ARF binds to E2F1.	bind
2241	1	1602	6	10	NULL	0	NULL	p19ARF	GP	endogenous	bind					E2F1	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_8_4455_s_151	11274364	( C) Endogenous p19ARF binds to E2F1.	bind
277	1	1603	5	10	NULL	0	NULL	PU.1	GP	endogenously expressed	bind					Dab2	GP			regulatory sequence	NULL		NULL	NULL	NULL	NULL	gw60_embo_21_3_211_s_63	11823414	( C) Endogenously expressed PU.1 binds to the Dab2 regulatory sequence.	bind
2242	1	1603	6	10	NULL	0	NULL	PU.1	GP	endogenously expressed	bind					Dab2	GP			regulatory sequence	NULL		NULL	NULL	NULL	NULL	gw60_embo_21_3_211_s_63	11823414	( C) Endogenously expressed PU.1 binds to the Dab2 regulatory sequence.	bind
278	1	1606	5	10	NULL	0	NULL	FGF-2	GP		bind					Namalwa-CD44vRA	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_111_8_1211_s_130	12697740	( c) Excess soluble heparin blocks the binding of FGF-2 to Namalwa-CD44vRA.	bind
2734	2	1606	5	10	NULL	0	NULL	heparin	GP	excess soluble	blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_111_8_1211_s_130	12697740	( c) Excess soluble heparin blocks the binding of FGF-2 to Namalwa-CD44vRA.	bind
2243	1	1606	6	10	NULL	0	NULL	FGF2	GP		bind					Namalwa-CD44vRA	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_111_8_1211_s_130	12697740	( c) Excess soluble heparin blocks the binding of FGF-2 to Namalwa-CD44vRA.	bind
2244	2	1606	6	10	NULL	0	NULL	heparin	GP	excess soluble	blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_111_8_1211_s_130	12697740	( c) Excess soluble heparin blocks the binding of FGF-2 to Namalwa-CD44vRA.	bind
280	1	1609	5	10	NULL	0	NULL	Ferritin	GP		bind				IRE	ACN	GP	purified	C517A		NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_18_10412_s_109	10468622	( C) Ferritin IRE binding activity of purified ACNC517A.	bind
2245	1	1609	6	10	NULL	0	NULL	Ferritin	GP		bind				IRE	ACN	GP	purified	C517A		NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_18_10412_s_109	10468622	( C) Ferritin IRE binding activity of purified ACNC517A.	bind
281	1	1610	5	10	NULL	0	NULL	FGF-2	GP		bind					Namalwa-CD44vRA	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_111_8_1211_s_156	12697740	( c) FGF-2 bound to Namalwa-CD44vRA induces enhanced proliferation of BaF-32 cells expressing  FGFR-1.	bind
282	2	1610	5	10	NULL	0	NULL	statement 1	Process		induce					BaF-32 cells	Cell	enhanced proliferation of			NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_111_8_1211_s_156	12697740	( c) FGF-2 bound to Namalwa-CD44vRA induces enhanced proliferation of BaF-32 cells expressing  FGFR-1.	bind
2735	3	1610	5	10	NULL	0	NULL	BaF-32 cells	Cell		express					FGFR-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_111_8_1211_s_156	12697740	( c) FGF-2 bound to Namalwa-CD44vRA induces enhanced proliferation of BaF-32 cells expressing  FGFR-1.	bind
2246	1	1610	6	10	NULL	0	NULL	FGF-2	GP		bind					Namalwa-CD44vRA	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_111_8_1211_s_156	12697740	( c) FGF-2 bound to Namalwa-CD44vRA induces enhanced proliferation of BaF-32 cells expressing  FGFR-1.	bind
2247	2	1610	6	10	NULL	0	NULL	BaF-32 cells	Cell		express					FGFR-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_111_8_1211_s_156	12697740	( c) FGF-2 bound to Namalwa-CD44vRA induces enhanced proliferation of BaF-32 cells expressing  FGFR-1.	bind
2248	3	1610	6	10	NULL	0	NULL	statement1	Process		induces					BaF-32 cells	Cell	enhanced proliferation of			NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_111_8_1211_s_156	12697740	( c) FGF-2 bound to Namalwa-CD44vRA induces enhanced proliferation of BaF-32 cells expressing  FGFR-1.	bind
283	1	1614	5	10	NULL	0	NULL	Five phenylalanine molecules	Chemical		bind					stimulatory complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_3_1212_s_104	11818540	( C) Five phenylalanine molecules bound to the stimulatory complex are depicted on the molecular surfaces of the GFRP pentamer with one GFRP monomer as a ribbon model (magenta).	bind
2249	1	1614	6	10	NULL	0	NULL	Five phenylalanine molecules	Chemical		bind					stimulatory complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_3_1212_s_104	11818540	( C) Five phenylalanine molecules bound to the stimulatory complex are depicted on the molecular surfaces of the GFRP pentamer with one GFRP monomer as a ribbon model (magenta).	bind
284	1	1615	5	10	NULL	0	NULL	p300	GP		bind					Smad3	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_10_2453_s_97	12743039	( C) Formation of a p300 - Smad3 - ZEB-1/deltaEF1 complex requires the binding of p300 to Smad3.	bind
285	2	1615	5	10	NULL	0	NULL	p300 - Smad3 - ZEB-1/deltaEF1	GP		forms					complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_10_2453_s_97	12743039	( C) Formation of a p300 - Smad3 - ZEB-1/deltaEF1 complex requires the binding of p300 to Smad3.	bind
286	3	1615	5	10	NULL	0	NULL	statement 2	Process		require					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_10_2453_s_97	12743039	( C) Formation of a p300 - Smad3 - ZEB-1/deltaEF1 complex requires the binding of p300 to Smad3.	bind
2300	1	1615	6	10	NULL	0	NULL	p300	GP		bind					Smad3	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_10_2453_s_97	12743039	( C) Formation of a p300 - Smad3 - ZEB-1/deltaEF1 complex requires the binding of p300 to Smad3.	bind
2301	2	1615	6	10	NULL	0	NULL	p300 - Smad3 - ZEB-1/deltaEF1	GP		forms 					complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_10_2453_s_97	12743039	( C) Formation of a p300 - Smad3 - ZEB-1/deltaEF1 complex requires the binding of p300 to Smad3.	bind
2302	3	1615	6	10	NULL	0	NULL	statement 2	Process		require					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_10_2453_s_97	12743039	( C) Formation of a p300 - Smad3 - ZEB-1/deltaEF1 complex requires the binding of p300 to Smad3.	bind
287	1	1616	5	10	NULL	0	NULL	hnRNP proteins	GP		bind					HIV	Organism			tat exon 2 ESS	NULL		NULL	NULL	NULL	NULL	gw60_embo_18_14_4060_s_54	10406810	( C) Further identification of hnRNP proteins that bind to the HIV  tat exon 2 ESS.	bind
2303	1	1616	6	10	NULL	0	NULL	hnRNP proteins	GP		bind					HIV	Organism			tat exon 2 ESS	NULL		NULL	NULL	NULL	NULL	gw60_embo_18_14_4060_s_54	10406810	( C) Further identification of hnRNP proteins that bind to the HIV  tat exon 2 ESS.	bind
2304	1	1617	6	10	NULL	0	NULL	GA	Chemical		bind					cell surface protein	GP	biotinylated			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_34_12095_s_103	16103367	( C) GA binds to a biotinylated cell surface protein.	bind
288	1	1618	5	10	NULL	0	NULL	GA	Chemical		bind					TfR	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_102_34_12095_s_132	16103367	( C) GA bound to TfR  in vitro can be displaced by active GA derivatives.	bind
289	2	1618	5	10	NULL	0	NULL	GA derivatives	Chemical		displaces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_34_12095_s_132	16103367	( C) GA bound to TfR  in vitro can be displaced by active GA derivatives.	bind
2305	1	1618	6	10	NULL	0	NULL	GA	Chemical		bind					TfR	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_102_34_12095_s_132	16103367	( C) GA bound to TfR  in vitro can be displaced by active GA derivatives.	bind
2306	2	1618	6	10	NULL	0	NULL	GA derivatives	Chemical	active	displaces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_34_12095_s_132	16103367	( C) GA bound to TfR  in vitro can be displaced by active GA derivatives.	bind
290	1	1619	5	10	NULL	0	NULL	Gab1	GP		bind			MBD		Grb2	GP		C-terminal SH3 domain		NULL	293 cells	NULL	NULL	NULL	NULL	gw60_pnas_98_11_6074_s_57	11353842	( C) Gab1 binds to the C-terminal SH3 domain of Grb2 through the MBD. 293 cells were transfected with the expression vector for Flag-tagged MBD of Gab1.	bind
2307	1	1619	6	10	NULL	0	NULL	Gab1	GP		bind			MBD		Grb2	GP		C-terminal SH3 domain		NULL	293 cells	NULL	NULL	NULL	NULL	gw60_pnas_98_11_6074_s_57	11353842	( C) Gab1 binds to the C-terminal SH3 domain of Grb2 through the MBD. 293 cells were transfected with the expression vector for Flag-tagged MBD of Gab1.	bind
291	1	1620	5	10	NULL	0	NULL	Ets-1	GP		bind					beta6 	GP			putative Ets sites in promoter	NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_115_2_339_s_72	15668738	( C) Gel mobility shift assay for Ets-1 binding to putative Ets sites in the beta6 promoter.	bind
2308	1	1620	6	10	NULL	0	NULL	Ets-1	GP		bind					beta6	GP			putative Ets sites of promoter	NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_115_2_339_s_72	15668738	( C) Gel mobility shift assay for Ets-1 binding to putative Ets sites in the beta6 promoter.	bind
292	1	1621	5	10	NULL	0	NULL	Rpp29	GP		bind					M1 RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_16_5120_s_243	16155184	( C) Gel shift analysis of binding of Rpp29 to M1 RNA.	bind
2309	1	1621	6	10	NULL	0	NULL	Rpp29	GP		bind					M1 RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_16_5120_s_243	16155184	( C) Gel shift analysis of binding of Rpp29 to M1 RNA.	bind
293	1	1622	5	10	NULL	0	NULL	GGA1	GP		bind			GAT domain		Arf1-GTP	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_20_0_153_s_248	15473838	( c) GGA1 GAT domain hook bound to Arf1-GTP (PDB ID 1J2J).	bind
2310	1	1622	6	10	NULL	0	NULL	GGA1	GP		bind			GAT domain		Arf1-GTP	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_20_0_153_s_248	15473838	( c) GGA1 GAT domain hook bound to Arf1-GTP (PDB ID 1J2J).	bind
2311	1	1623	6	10	NULL	0	NULL	nuclear proteins	GP		bind									dfd-1 element	NULL	body axis	NULL	NULL	NULL	NULL	gw60_pnas_96_4_1445_s_147	9990043	( C) Gradient of nuclear proteins binding to the dfd-1 element along the body axis with sharp decrease of DNA-protein interactions in TFZ and head tissue.	bind
2312	2	1623	6	10	NULL	0	NULL	DNA	NucleicAcid		interacts with					protein	GP				NULL	TFZ 	NULL	NULL	NULL	NULL	gw60_pnas_96_4_1445_s_147	9990043	( C) Gradient of nuclear proteins binding to the dfd-1 element along the body axis with sharp decrease of DNA-protein interactions in TFZ and head tissue.	bind
52614	3	1623	6	10	NULL	0	NULL	DNA	NucleicAcid		interacts with					protein	GP				NULL	head tissue	NULL	NULL	NULL	NULL	gw60_pnas_96_4_1445_s_147	9990043	( C) Gradient of nuclear proteins binding to the dfd-1 element along the body axis with sharp decrease of DNA-protein interactions in TFZ and head tissue.	bind
52615	4	1623	6	10	NULL	0	NULL	statement 1	Process		decrease					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_4_1445_s_147	9990043	( C) Gradient of nuclear proteins binding to the dfd-1 element along the body axis with sharp decrease of DNA-protein interactions in TFZ and head tissue.	bind
52616	5	1623	6	10	NULL	0	NULL	statement 1	Process		decrease					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_4_1445_s_147	9990043	( C) Gradient of nuclear proteins binding to the dfd-1 element along the body axis with sharp decrease of DNA-protein interactions in TFZ and head tissue.	bind
3112	1	1624	5	10	NULL	0	NULL	Elk	GP		bind			1-93		Elk-1	GP		B-box		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_20_5666_s_142	10523309	( C) GST pull-down assay of binding of Elk1-93 to GST fusion proteins containing the Elk-1 B-box or D-domain in the absence (lanes 1 and 3) or presence (lanes 2 and 4) of B-box competitor peptide (7 muM).	bind
3114	2	1624	5	10	NULL	0	NULL	Elk	GP		bind			1-93		Elk-1	GP		D-domain		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_20_5666_s_142	10523309	( C) GST pull-down assay of binding of Elk1-93 to GST fusion proteins containing the Elk-1 B-box or D-domain in the absence (lanes 1 and 3) or presence (lanes 2 and 4) of B-box competitor peptide (7 muM).	bind
2313	1	1624	6	10	NULL	0	NULL	Elk	GP		bind			1-93		ELk-1	GP		B-box		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_20_5666_s_142	10523309	( C) GST pull-down assay of binding of Elk1-93 to GST fusion proteins containing the Elk-1 B-box or D-domain in the absence (lanes 1 and 3) or presence (lanes 2 and 4) of B-box competitor peptide (7 muM).	bind
2314	2	1624	6	10	NULL	0	NULL	Elk	GP		bind			1-93		ELk-1	GP		D-domain		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_20_5666_s_142	10523309	( C) GST pull-down assay of binding of Elk1-93 to GST fusion proteins containing the Elk-1 B-box or D-domain in the absence (lanes 1 and 3) or presence (lanes 2 and 4) of B-box competitor peptide (7 muM).	bind
295	1	1625	5	10	NULL	0	NULL	GST-cyclin E-Cdk2	GP		bind					Fbw7	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_294_5540_173_s_48	11533444	( C) GST-cyclin E-Cdk2 binds Fbw7.	bind
2315	1	1625	6	10	NULL	0	NULL	GST-cyclin E-Cdk2	GP		bind					Fbw7	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_294_5540_173_s_48	11533444	( C) GST-cyclin E-Cdk2 binds Fbw7.	bind
296	1	1626	5	10	NULL	0	NULL	GST-DSCR1/calcineurin	GP		bind					FK506/FKBP12	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_13_1595_s_76	10887154	( C) GST-DSCR1/calcineurin bound to FK506/FKBP12 in the presence of calmodulin and 2 mM CaCl2.	bind
3147	2	1626	5	10	NULL	0	NULL	statement 1	Process		in the presence of					calmodulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_13_1595_s_76	10887154	( C) GST-DSCR1/calcineurin bound to FK506/FKBP12 in the presence of calmodulin and 2 mM CaCl2.	bind
3148	3	1626	5	10	NULL	0	NULL	statement 1	Process		in the presence of					CaCl2	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_13_1595_s_76	10887154	( C) GST-DSCR1/calcineurin bound to FK506/FKBP12 in the presence of calmodulin and 2 mM CaCl2.	bind
2316	1	1626	6	10	NULL	0	NULL	GST-DSCR1/calcineurin	GP		bind					FK506/FKBP12	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_13_1595_s_76	10887154	( C) GST-DSCR1/calcineurin bound to FK506/FKBP12 in the presence of calmodulin and 2 mM CaCl2.	bind
2317	2	1626	6	10	NULL	0	NULL	statement 1	Process		in presence of 					calmodulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_13_1595_s_76	10887154	( C) GST-DSCR1/calcineurin bound to FK506/FKBP12 in the presence of calmodulin and 2 mM CaCl2.	bind
2318	3	1626	6	10	NULL	0	NULL	statement 1	Process		in presence of 					CaCl2	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_13_1595_s_76	10887154	( C) GST-DSCR1/calcineurin bound to FK506/FKBP12 in the presence of calmodulin and 2 mM CaCl2.	bind
297	1	1628	5	10	NULL	0	NULL	Gst-IsdC	GP		bind		 dose-dependently			heme-agarose beads	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_science_299_5608_906_s_56	12574635	( C) Gst-IsdC binds heme-agarose beads in a dose-dependent manner and incubation with  heme-iron abolishes this binding.	bind
298	2	1628	5	10	NULL	0	NULL	heme-iron 	Chemical		abolish					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_science_299_5608_906_s_56	12574635	( C) Gst-IsdC binds heme-agarose beads in a dose-dependent manner and incubation with  heme-iron abolishes this binding.	bind
2320	1	1628	6	10	NULL	0	NULL	Gst-IsdC	GP		bind		dose-dependently			heme-agarose beads	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_science_299_5608_906_s_56	12574635	( C) Gst-IsdC binds heme-agarose beads in a dose-dependent manner and incubation with  heme-iron abolishes this binding.	bind
2321	2	1628	6	10	NULL	0	NULL	heme-iron	Chemical		abolishes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_science_299_5608_906_s_56	12574635	( C) Gst-IsdC binds heme-agarose beads in a dose-dependent manner and incubation with  heme-iron abolishes this binding.	bind
299	1	1630	5	10	NULL	0	NULL	GTP	Chemical		bind		specifically			CIITA	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_285_5432_1402_s_53	10464099	( C) GTP binding by CIITA is specific.	bind
2322	1	1630	6	10	NULL	0	NULL	GTP	Chemical		bind		specifically			CIITA	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_285_5432_1402_s_53	10464099	( C) GTP binding by CIITA is specific.	bind
300	1	1631	5	10	NULL	0	NULL	MukF	GP	His-tagged	bind			302-440		MukE	GP		1-209		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_11_1921_s_139	15902272	( C) His-tagged MukF(302 440) binds MukE(1 209).	bind
2323	1	1631	6	10	NULL	0	NULL	MukF	GP	His-tagged	bind			302-440		MukE	GP		1-209		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_11_1921_s_139	15902272	( C) His-tagged MukF(302 440) binds MukE(1 209).	bind
896	1	1633	5	10	NULL	0	NULL				bind			F302W		mAb 7E3	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_143_6_1523_s_261	9852148	( C) Histograms (mean  plus-or-minus  SEM,  n = 4)  showing a gain of F302W  binding to mAb 7E3 and a loss  of T209A binding to this mAb.	bind
897	2	1633	5	10	NULL	0	NULL				bind			T209A		mAb 7E3	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_143_6_1523_s_261	9852148	( C) Histograms (mean  plus-or-minus  SEM,  n = 4)  showing a gain of F302W  binding to mAb 7E3 and a loss  of T209A binding to this mAb.	bind
2324	1	1633	6	10	NULL	0	NULL				bind			F302W		mAb 7E3	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_143_6_1523_s_261	9852148	( C) Histograms (mean  plus-or-minus  SEM,  n = 4)  showing a gain of F302W  binding to mAb 7E3 and a loss  of T209A binding to this mAb.	bind
2325	2	1633	6	10	NULL	0	NULL				bind			T209A		mAb 7E3	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_143_6_1523_s_261	9852148	( C) Histograms (mean  plus-or-minus  SEM,  n = 4)  showing a gain of F302W  binding to mAb 7E3 and a loss  of T209A binding to this mAb.	bind
301	1	1634	5	10	NULL	0	NULL	hRAP74cc	GP		bind					GST-hFCP1pep	GP		941-961		NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_5_2296_s_26	12591941	( c) hRAP74cc binding to GST-hFCP1pep (941-961).	bind
2326	1	1634	6	10	NULL	0	NULL	RAP74cc	GP	human	bind					GST-FCP1pep	GP	human	941-961		NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_5_2296_s_26	12591941	( c) hRAP74cc binding to GST-hFCP1pep (941-961).	bind
302	1	1635	5	10	NULL	0	NULL	Hrr25p	GP		phosphorylate					Crz1p	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_genesdev_17_21_2698_s_52	14597664	( C) Hrr25p phosphorylates and binds to Crz1p in vivo.	bind
303	2	1635	5	10	NULL	0	NULL	Hrr25p	GP		bind					Crz1p	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_genesdev_17_21_2698_s_52	14597664	( C) Hrr25p phosphorylates and binds to Crz1p in vivo.	bind
2327	1	1635	6	10	NULL	0	NULL	Hrr25p	GP		phosphorylates					Crz1p	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_genesdev_17_21_2698_s_52	14597664	( C) Hrr25p phosphorylates and binds to Crz1p in vivo.	bind
2328	2	1635	6	10	NULL	0	NULL	Hrr25p	GP		bind					Crz1p	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_genesdev_17_21_2698_s_52	14597664	( C) Hrr25p phosphorylates and binds to Crz1p in vivo.	bind
304	1	1636	5	10	NULL	0	NULL	HuR protein	GP		bind					p27 	GP			5'UTR	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_23_3087_s_135	12464637	( C) HuR protein binds to the p27 5'UTR.	bind
2329	1	1636	6	10	NULL	0	NULL	HuR protein	GP		bind					p27	GP			5' UTR	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_23_3087_s_135	12464637	( C) HuR protein binds to the p27 5'UTR.	bind
305	1	1637	5	10	NULL	0	NULL	ICE1	GP		bind		strongly			MYC-2 DNA fragment	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_8_1043_s_168	12672693	( C) ICE1 binds to the MYC-2 DNA fragment more strongly than to the other DNA fragments.	bind
2343	1	1637	6	10	NULL	0	NULL	ICE1	GP		bind		strongly			MYC-2 DNA fragment	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_8_1043_s_168	12672693	( C) ICE1 binds to the MYC-2 DNA fragment more strongly than to the other DNA fragments.	bind
306	1	1638	5	10	NULL	0	NULL	ICSBP	GP		bind					Dab2	GP			promoter	NULL	myeloid progenitor cells	NULL	NULL	NULL	NULL	gw60_embo_21_3_211_s_100	11823414	( C) ICSBP and PU.1 bind to the Dab2 promoter in myeloid progenitor cells.	bind
3149	2	1638	5	10	NULL	0	NULL	PU.1	GP		bind					Dab2	GP			promoter	NULL	myeloid progenitor cells	NULL	NULL	NULL	NULL	gw60_embo_21_3_211_s_100	11823414	( C) ICSBP and PU.1 bind to the Dab2 promoter in myeloid progenitor cells.	bind
2358	1	1638	6	10	NULL	0	NULL	ICSBP	GP		bind					Dab2	GP			promoter	NULL	myeloid progenitor cells	NULL	NULL	NULL	NULL	gw60_embo_21_3_211_s_100	11823414	( C) ICSBP and PU.1 bind to the Dab2 promoter in myeloid progenitor cells.	bind
2359	2	1638	6	10	NULL	0	NULL	PU.1	GP		bind					Dab2	GP			promoter	NULL	myeloid progenitor cells	NULL	NULL	NULL	NULL	gw60_embo_21_3_211_s_100	11823414	( C) ICSBP and PU.1 bind to the Dab2 promoter in myeloid progenitor cells.	bind
307	1	1640	5	10	NULL	0	NULL	ICSBP	GP		bind					Dab2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_21_3_211_s_116	11823414	( C) IFN-gamma induces ICSBP binding to the Dab2 promoter.	bind
308	2	1640	5	10	NULL	0	NULL	IFN-gamma	GP		induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_3_211_s_116	11823414	( C) IFN-gamma induces ICSBP binding to the Dab2 promoter.	bind
2360	1	1640	6	10	NULL	0	NULL	ICSBP	GP		bind					Dab2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_21_3_211_s_116	11823414	( C) IFN-gamma induces ICSBP binding to the Dab2 promoter.	bind
2361	2	1640	6	10	NULL	0	NULL	IFN-gamma	GP		induces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_3_211_s_116	11823414	( C) IFN-gamma induces ICSBP binding to the Dab2 promoter.	bind
309	1	1641	5	10	NULL	0	NULL	Ikaros	GP		bind					lambda5 	GP			Ik-2 site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_20_11_2812_s_62	11387214	( C) Ikaros and Aiolos bind to the Ik-2 site of the lambda5 promoter.	bind
310	2	1641	5	10	NULL	0	NULL	Aiolos	GP		bind					lambda5	GP			Ik-2 site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_20_11_2812_s_62	11387214	( C) Ikaros and Aiolos bind to the Ik-2 site of the lambda5 promoter.	bind
2362	1	1641	6	10	NULL	0	NULL	Ikaros	GP		bind					lambda5	GP			Ik-2 site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_20_11_2812_s_62	11387214	( C) Ikaros and Aiolos bind to the Ik-2 site of the lambda5 promoter.	bind
2363	2	1641	6	10	NULL	0	NULL	Aiolos	GP		bind					lambda5	GP			Ik-2 site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_20_11_2812_s_62	11387214	( C) Ikaros and Aiolos bind to the Ik-2 site of the lambda5 promoter.	bind
318	1	1642	5	10	NULL	0	NULL	Gbeta1	Chemical		bind					GIRK-GST	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_17_9771_s_114	10944236	( C) Immunoblots from GST pull down assays with Gbetacommon (betac) and gamma2 antisera demonstrate binding of beta1 ( 1), beta3 ( 3), and beta4 ( 4), as well as gamma2, to each of the GIRK-GST fusion proteins; Gbetagamma subunits did not bind to GST alone.	bind
319	2	1642	5	10	NULL	0	NULL	Gbeta3	Chemical		bind					GIRK-GST	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_17_9771_s_114	10944236	( C) Immunoblots from GST pull down assays with Gbetacommon (betac) and gamma2 antisera demonstrate binding of beta1 ( 1), beta3 ( 3), and beta4 ( 4), as well as gamma2, to each of the GIRK-GST fusion proteins; Gbetagamma subunits did not bind to GST alone.	bind
320	3	1642	5	10	NULL	0	NULL	Gbeta4	Chemical		bind					GIRK-GST	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_17_9771_s_114	10944236	( C) Immunoblots from GST pull down assays with Gbetacommon (betac) and gamma2 antisera demonstrate binding of beta1 ( 1), beta3 ( 3), and beta4 ( 4), as well as gamma2, to each of the GIRK-GST fusion proteins; Gbetagamma subunits did not bind to GST alone.	bind
321	4	1642	5	10	NULL	0	NULL	Ggamma2	Chemical		bind					GIRK-GST	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_17_9771_s_114	10944236	( C) Immunoblots from GST pull down assays with Gbetacommon (betac) and gamma2 antisera demonstrate binding of beta1 ( 1), beta3 ( 3), and beta4 ( 4), as well as gamma2, to each of the GIRK-GST fusion proteins; Gbetagamma subunits did not bind to GST alone.	bind
3322	5	1642	5	10	NULL	0	NULL	Gbeta1	Chemical		does not bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_17_9771_s_114	10944236	( C) Immunoblots from GST pull down assays with Gbetacommon (betac) and gamma2 antisera demonstrate binding of beta1 ( 1), beta3 ( 3), and beta4 ( 4), as well as gamma2, to each of the GIRK-GST fusion proteins; Gbetagamma subunits did not bind to GST alone.	bind
3323	6	1642	5	10	NULL	0	NULL	Gbeta3	Chemical		does not bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_17_9771_s_114	10944236	( C) Immunoblots from GST pull down assays with Gbetacommon (betac) and gamma2 antisera demonstrate binding of beta1 ( 1), beta3 ( 3), and beta4 ( 4), as well as gamma2, to each of the GIRK-GST fusion proteins; Gbetagamma subunits did not bind to GST alone.	bind
3324	7	1642	5	10	NULL	0	NULL	Gbeta4	Chemical		does not bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_17_9771_s_114	10944236	( C) Immunoblots from GST pull down assays with Gbetacommon (betac) and gamma2 antisera demonstrate binding of beta1 ( 1), beta3 ( 3), and beta4 ( 4), as well as gamma2, to each of the GIRK-GST fusion proteins; Gbetagamma subunits did not bind to GST alone.	bind
3325	8	1642	5	10	NULL	0	NULL	Ggamma2	Chemical		does not bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_17_9771_s_114	10944236	( C) Immunoblots from GST pull down assays with Gbetacommon (betac) and gamma2 antisera demonstrate binding of beta1 ( 1), beta3 ( 3), and beta4 ( 4), as well as gamma2, to each of the GIRK-GST fusion proteins; Gbetagamma subunits did not bind to GST alone.	bind
46156	9	1642	5	10	NULL	0	NULL	GIRK-GST	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_17_9771_s_114	10944236	( C) Immunoblots from GST pull down assays with Gbetacommon (betac) and gamma2 antisera demonstrate binding of beta1 ( 1), beta3 ( 3), and beta4 ( 4), as well as gamma2, to each of the GIRK-GST fusion proteins; Gbetagamma subunits did not bind to GST alone.	bind
2364	1	1642	6	10	NULL	0	NULL	GIRK-GST	GP		bind					Gbeta1	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_17_9771_s_114	10944236	( C) Immunoblots from GST pull down assays with Gbetacommon (betac) and gamma2 antisera demonstrate binding of beta1 ( 1), beta3 ( 3), and beta4 ( 4), as well as gamma2, to each of the GIRK-GST fusion proteins; Gbetagamma subunits did not bind to GST alone.	bind
2365	2	1642	6	10	NULL	0	NULL	GIRK-GST	GP		bind					Gbeta3	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_17_9771_s_114	10944236	( C) Immunoblots from GST pull down assays with Gbetacommon (betac) and gamma2 antisera demonstrate binding of beta1 ( 1), beta3 ( 3), and beta4 ( 4), as well as gamma2, to each of the GIRK-GST fusion proteins; Gbetagamma subunits did not bind to GST alone.	bind
2366	3	1642	6	10	NULL	0	NULL	GIRK-GST	GP		bind					Gbeta4	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_17_9771_s_114	10944236	( C) Immunoblots from GST pull down assays with Gbetacommon (betac) and gamma2 antisera demonstrate binding of beta1 ( 1), beta3 ( 3), and beta4 ( 4), as well as gamma2, to each of the GIRK-GST fusion proteins; Gbetagamma subunits did not bind to GST alone.	bind
2367	4	1642	6	10	NULL	0	NULL	GIRK-GST	GP		bind					Ggamma2	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_17_9771_s_114	10944236	( C) Immunoblots from GST pull down assays with Gbetacommon (betac) and gamma2 antisera demonstrate binding of beta1 ( 1), beta3 ( 3), and beta4 ( 4), as well as gamma2, to each of the GIRK-GST fusion proteins; Gbetagamma subunits did not bind to GST alone.	bind
2368	5	1642	6	10	NULL	0	NULL	Gbeta1	Chemical		does not bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_17_9771_s_114	10944236	( C) Immunoblots from GST pull down assays with Gbetacommon (betac) and gamma2 antisera demonstrate binding of beta1 ( 1), beta3 ( 3), and beta4 ( 4), as well as gamma2, to each of the GIRK-GST fusion proteins; Gbetagamma subunits did not bind to GST alone.	bind
2369	6	1642	6	10	NULL	0	NULL	Gbeta3	Chemical		does not bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_17_9771_s_114	10944236	( C) Immunoblots from GST pull down assays with Gbetacommon (betac) and gamma2 antisera demonstrate binding of beta1 ( 1), beta3 ( 3), and beta4 ( 4), as well as gamma2, to each of the GIRK-GST fusion proteins; Gbetagamma subunits did not bind to GST alone.	bind
2370	7	1642	6	10	NULL	0	NULL	Gbeta4	Chemical		does not bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_17_9771_s_114	10944236	( C) Immunoblots from GST pull down assays with Gbetacommon (betac) and gamma2 antisera demonstrate binding of beta1 ( 1), beta3 ( 3), and beta4 ( 4), as well as gamma2, to each of the GIRK-GST fusion proteins; Gbetagamma subunits did not bind to GST alone.	bind
2371	8	1642	6	10	NULL	0	NULL	Ggamma2	Chemical		does not bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_17_9771_s_114	10944236	( C) Immunoblots from GST pull down assays with Gbetacommon (betac) and gamma2 antisera demonstrate binding of beta1 ( 1), beta3 ( 3), and beta4 ( 4), as well as gamma2, to each of the GIRK-GST fusion proteins; Gbetagamma subunits did not bind to GST alone.	bind
46177	9	1642	6	10	NULL	0	NULL	GST-GIRK	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_17_9771_s_114	10944236	( C) Immunoblots from GST pull down assays with Gbetacommon (betac) and gamma2 antisera demonstrate binding of beta1 ( 1), beta3 ( 3), and beta4 ( 4), as well as gamma2, to each of the GIRK-GST fusion proteins; Gbetagamma subunits did not bind to GST alone.	bind
322	1	1643	5	10	NULL	0	NULL	MAGI-2	GP		bind					GST - nephrin	GP		tail		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_28_9814_s_97	15994232	( C) Immunoblotting with anti-MAGI-2/S-SCAM IgG and anti-MAGI-2 IgG showed that MAGI-2  binds to GST - nephrin tail (lane 1) but not to GST alone (lane 2).	bind
3152	2	1643	5	10	NULL	0	NULL	MAGI-2	GP		does not bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_28_9814_s_97	15994232	( C) Immunoblotting with anti-MAGI-2/S-SCAM IgG and anti-MAGI-2 IgG showed that MAGI-2  binds to GST - nephrin tail (lane 1) but not to GST alone (lane 2).	bind
2372	1	1643	6	10	NULL	0	NULL	MAGI-2	GP		bind					GST-nephrin	GP		tail		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_28_9814_s_97	15994232	( C) Immunoblotting with anti-MAGI-2/S-SCAM IgG and anti-MAGI-2 IgG showed that MAGI-2  binds to GST - nephrin tail (lane 1) but not to GST alone (lane 2).	bind
2373	2	1643	6	10	NULL	0	NULL	MAGI-2	GP		does not bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_28_9814_s_97	15994232	( C) Immunoblotting with anti-MAGI-2/S-SCAM IgG and anti-MAGI-2 IgG showed that MAGI-2  binds to GST - nephrin tail (lane 1) but not to GST alone (lane 2).	bind
323	1	1644	5	10	NULL	0	NULL	Pho4	GP	unphosphorylated	bind					Pse1	GP				NULL		NULL	NULL	NULL	NULL	gw60_annurevcelldevbiol_15_0_291_s_104	10611964	( c) In   low-phosphate conditions unphosphorylated Pho4 binds to   its import receptor, Pse1, and is translocated   into the nucleus.	bind
324	2	1644	5	10	NULL	0	NULL	statement 1	Process		translocated to					nucleus	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_annurevcelldevbiol_15_0_291_s_104	10611964	( c) In   low-phosphate conditions unphosphorylated Pho4 binds to   its import receptor, Pse1, and is translocated   into the nucleus.	bind
2883	3	1644	5	10	NULL	0	NULL	statement 1	Process		occurs in					low-phosphate conditions	Process				NULL		NULL	NULL	NULL	NULL	gw60_annurevcelldevbiol_15_0_291_s_104	10611964	( c) In   low-phosphate conditions unphosphorylated Pho4 binds to   its import receptor, Pse1, and is translocated   into the nucleus.	bind
46157	4	1644	5	10	NULL	0	NULL	Pse1	GP		is a type of					import receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_annurevcelldevbiol_15_0_291_s_104	10611964	( c) In   low-phosphate conditions unphosphorylated Pho4 binds to   its import receptor, Pse1, and is translocated   into the nucleus.	bind
52622	5	1644	5	10	NULL	0	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_annurevcelldevbiol_15_0_291_s_104	10611964	( c) In   low-phosphate conditions unphosphorylated Pho4 binds to   its import receptor, Pse1, and is translocated   into the nucleus.	bind
2374	1	1644	6	10	NULL	0	NULL	Pho4	GP	unphosphorylated	bind					Pse1	GP				NULL		NULL	NULL	NULL	NULL	gw60_annurevcelldevbiol_15_0_291_s_104	10611964	( c) In   low-phosphate conditions unphosphorylated Pho4 binds to   its import receptor, Pse1, and is translocated   into the nucleus.	bind
2375	2	1644	6	10	NULL	0	NULL	statement 1	Process		occurs in					low-phosphate conditions	Process				NULL		NULL	NULL	NULL	NULL	gw60_annurevcelldevbiol_15_0_291_s_104	10611964	( c) In   low-phosphate conditions unphosphorylated Pho4 binds to   its import receptor, Pse1, and is translocated   into the nucleus.	bind
2376	3	1644	6	10	NULL	0	NULL	Pho4	GP	unphosphorylated	translocated to					nucleus	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_annurevcelldevbiol_15_0_291_s_104	10611964	( c) In   low-phosphate conditions unphosphorylated Pho4 binds to   its import receptor, Pse1, and is translocated   into the nucleus.	bind
2377	4	1644	6	10	NULL	0	NULL	statement 1	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_annurevcelldevbiol_15_0_291_s_104	10611964	( c) In   low-phosphate conditions unphosphorylated Pho4 binds to   its import receptor, Pse1, and is translocated   into the nucleus.	bind
46179	5	1644	6	10	NULL	0	NULL	Pse1	GP		is a type of					import receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_annurevcelldevbiol_15_0_291_s_104	10611964	( c) In   low-phosphate conditions unphosphorylated Pho4 binds to   its import receptor, Pse1, and is translocated   into the nucleus.	bind
325	1	1645	5	10	NULL	0	NULL	T cells	Cell	activated	decrease					Bcl-2	GP	levels of			NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_22_0_765_s_231	15032596	( C) In activated T cells levels of Bcl-2 fall, and consequently less of the Bim protein  is bound to Bcl-2.	bind
326	2	1645	5	10	NULL	0	NULL	Bim protein	GP		bind					Bcl-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_22_0_765_s_231	15032596	( C) In activated T cells levels of Bcl-2 fall, and consequently less of the Bim protein  is bound to Bcl-2.	bind
327	3	1645	5	10	NULL	0	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_22_0_765_s_231	15032596	( C) In activated T cells levels of Bcl-2 fall, and consequently less of the Bim protein  is bound to Bcl-2.	bind
2378	1	1645	6	10	NULL	0	NULL	Bim protein	GP		bind					Bcl-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_22_0_765_s_231	15032596	( C) In activated T cells levels of Bcl-2 fall, and consequently less of the Bim protein  is bound to Bcl-2.	bind
2379	2	1645	6	10	NULL	0	NULL	T cells	Cell	activated	decreases					Bcl-2	GP	levels of 			NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_22_0_765_s_231	15032596	( C) In activated T cells levels of Bcl-2 fall, and consequently less of the Bim protein  is bound to Bcl-2.	bind
2380	3	1645	6	10	NULL	0	NULL	statement 2	Process		leads to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_22_0_765_s_231	15032596	( C) In activated T cells levels of Bcl-2 fall, and consequently less of the Bim protein  is bound to Bcl-2.	bind
328	1	1646	5	10	NULL	0	NULL	Cdc42p	GP		bind					Gic2p	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_18_5360_s_183	9736614	( C) In contrast to Gic2p-N1-208,  cdc4-1 cells overexpressing Gic2p-crib- from the  GAL promoter at 30 degrees C were viable, confirming that binding of Cdc42p to Gic2p is required for its function (Brown  et al., 1997  ).	bind
3153	2	1646	5	10	NULL	0	NULL	cdc4-1 cells	Cell		overexpress					Gic2p-crib-	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_18_5360_s_183	9736614	( C) In contrast to Gic2p-N1-208,  cdc4-1 cells overexpressing Gic2p-crib- from the  GAL promoter at 30 degrees C were viable, confirming that binding of Cdc42p to Gic2p is required for its function (Brown  et al., 1997  ).	bind
3157	3	1646	5	10	NULL	0	NULL	statement 1	Process		is required for					Gic2p	GP	function of			NULL		NULL	NULL	NULL	NULL	gw60_embo_17_18_5360_s_183	9736614	( C) In contrast to Gic2p-N1-208,  cdc4-1 cells overexpressing Gic2p-crib- from the  GAL promoter at 30 degrees C were viable, confirming that binding of Cdc42p to Gic2p is required for its function (Brown  et al., 1997  ).	bind
3159	4	1646	5	10	NULL	0	NULL	statement 1	Process		is required for					cdc4-1 cells	Cell	function of			NULL		NULL	NULL	NULL	NULL	gw60_embo_17_18_5360_s_183	9736614	( C) In contrast to Gic2p-N1-208,  cdc4-1 cells overexpressing Gic2p-crib- from the  GAL promoter at 30 degrees C were viable, confirming that binding of Cdc42p to Gic2p is required for its function (Brown  et al., 1997  ).	bind
2381	1	1646	6	10	NULL	0	NULL	Cdc42p	GP		bind					Gic2p	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_18_5360_s_183	9736614	( C) In contrast to Gic2p-N1-208,  cdc4-1 cells overexpressing Gic2p-crib- from the  GAL promoter at 30 degrees C were viable, confirming that binding of Cdc42p to Gic2p is required for its function (Brown  et al., 1997  ).	bind
2382	2	1646	6	10	NULL	0	NULL	cdc4-1 cells	Cell		overexpress					Gic2p-crib-	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_18_5360_s_183	9736614	( C) In contrast to Gic2p-N1-208,  cdc4-1 cells overexpressing Gic2p-crib- from the  GAL promoter at 30 degrees C were viable, confirming that binding of Cdc42p to Gic2p is required for its function (Brown  et al., 1997  ).	bind
2476	3	1646	6	10	NULL	0	NULL	statement 1	Process		is required for					Gic2p	GP	function of 			NULL		NULL	NULL	NULL	NULL	gw60_embo_17_18_5360_s_183	9736614	( C) In contrast to Gic2p-N1-208,  cdc4-1 cells overexpressing Gic2p-crib- from the  GAL promoter at 30 degrees C were viable, confirming that binding of Cdc42p to Gic2p is required for its function (Brown  et al., 1997  ).	bind
2477	4	1646	6	10	NULL	0	NULL	statement 1	Process		is required for					cdc4-1 cells	Cell	function of			NULL		NULL	NULL	NULL	NULL	gw60_embo_17_18_5360_s_183	9736614	( C) In contrast to Gic2p-N1-208,  cdc4-1 cells overexpressing Gic2p-crib- from the  GAL promoter at 30 degrees C were viable, confirming that binding of Cdc42p to Gic2p is required for its function (Brown  et al., 1997  ).	bind
329	1	1647	5	10	NULL	0	NULL	PDK1	GP		bind					PKB	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_16_4380_s_254	11500365	( C) In contrast, the PIF-binding pocket of PDK1 is not involved in the binding of PDK1 to PKB.	bind
330	2	1647	5	10	NULL	0	NULL	PDK1	GP		not involved in			PIF-binding pocket		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_16_4380_s_254	11500365	( C) In contrast, the PIF-binding pocket of PDK1 is not involved in the binding of PDK1 to PKB.	bind
2383	1	1647	6	10	NULL	0	NULL	PDK1	GP		bind					PKB	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_16_4380_s_254	11500365	( C) In contrast, the PIF-binding pocket of PDK1 is not involved in the binding of PDK1 to PKB.	bind
2384	2	1647	6	10	NULL	0	NULL	PDK1	GP		is not involved in			PIF-binding pocket		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_16_4380_s_254	11500365	( C) In contrast, the PIF-binding pocket of PDK1 is not involved in the binding of PDK1 to PKB.	bind
379	1	1648	5	10	NULL	0	NULL	PrPC	GP	mutant	bind					protein X	GP				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_67_0_793_s_95	9759504	( C) In inherited disease and perhaps   with spontaneous disease in the presence of a somatic cell mutation,   mutant PrPC can bind protein X and form the PrP*/X/PrP*/X   encounter complex, which can then form PrPSc/ut in the absence of a PrPSc template.	bind
381	2	1648	5	10	NULL	0	NULL	statement 1	Process		forms					PrP*/X/PrP*/X encounter complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_67_0_793_s_95	9759504	( C) In inherited disease and perhaps   with spontaneous disease in the presence of a somatic cell mutation,   mutant PrPC can bind protein X and form the PrP*/X/PrP*/X   encounter complex, which can then form PrPSc/ut in the absence of a PrPSc template.	bind
383	3	1648	5	10	NULL	0	NULL	statement 2	Process		forms					PrPSc/ut	GP				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_67_0_793_s_95	9759504	( C) In inherited disease and perhaps   with spontaneous disease in the presence of a somatic cell mutation,   mutant PrPC can bind protein X and form the PrP*/X/PrP*/X   encounter complex, which can then form PrPSc/ut in the absence of a PrPSc template.	bind
45935	4	1648	5	10	NULL	0	NULL	statement 3	Process		in the absence of					PrPSc template	GP				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_67_0_793_s_95	9759504	( C) In inherited disease and perhaps   with spontaneous disease in the presence of a somatic cell mutation,   mutant PrPC can bind protein X and form the PrP*/X/PrP*/X   encounter complex, which can then form PrPSc/ut in the absence of a PrPSc template.	bind
2471	1	1648	6	10	NULL	0	NULL	PrPC	GP	mutant	bind					protein X	GP				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_67_0_793_s_95	9759504	( C) In inherited disease and perhaps   with spontaneous disease in the presence of a somatic cell mutation,   mutant PrPC can bind protein X and form the PrP*/X/PrP*/X   encounter complex, which can then form PrPSc/ut in the absence of a PrPSc template.	bind
2472	2	1648	6	10	NULL	0	NULL	statement 1	Process		forms					PrP*/X/PrP*/X encounter complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_67_0_793_s_95	9759504	( C) In inherited disease and perhaps   with spontaneous disease in the presence of a somatic cell mutation,   mutant PrPC can bind protein X and form the PrP*/X/PrP*/X   encounter complex, which can then form PrPSc/ut in the absence of a PrPSc template.	bind
2473	3	1648	6	10	NULL	0	NULL	PrP*/X/PrP*/X encounter complex	GP		forms					PrPSc/ut 	GP				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_67_0_793_s_95	9759504	( C) In inherited disease and perhaps   with spontaneous disease in the presence of a somatic cell mutation,   mutant PrPC can bind protein X and form the PrP*/X/PrP*/X   encounter complex, which can then form PrPSc/ut in the absence of a PrPSc template.	bind
2474	4	1648	6	10	NULL	0	NULL	statement 3	Process		 in absence of 					PrPSc template	GP				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_67_0_793_s_95	9759504	( C) In inherited disease and perhaps   with spontaneous disease in the presence of a somatic cell mutation,   mutant PrPC can bind protein X and form the PrP*/X/PrP*/X   encounter complex, which can then form PrPSc/ut in the absence of a PrPSc template.	bind
384	1	1649	5	10	NULL	0	NULL	Pho4	GP	unphosphorylated	bind					Pse1	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_15_0_291_s_120	10611964	( c) In low-phosphate conditions unphosphorylated Pho4 binds to its import receptor,  Pse1, and is translocated into the nucleus.	bind
385	2	1649	5	10	NULL	0	NULL	statement 1	Process		translocated to					nucleus	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_15_0_291_s_120	10611964	( c) In low-phosphate conditions unphosphorylated Pho4 binds to its import receptor,  Pse1, and is translocated into the nucleus.	bind
2885	3	1649	5	10	NULL	0	NULL	statement 1	Process		occurs in					low-phosphate conditions	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_15_0_291_s_120	10611964	( c) In low-phosphate conditions unphosphorylated Pho4 binds to its import receptor,  Pse1, and is translocated into the nucleus.	bind
52623	4	1649	5	10	NULL	0	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_15_0_291_s_120	10611964	( c) In low-phosphate conditions unphosphorylated Pho4 binds to its import receptor,  Pse1, and is translocated into the nucleus.	bind
52624	5	1649	5	10	NULL	0	NULL	Pse1	GP		is a type of					import receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_15_0_291_s_120	10611964	( c) In low-phosphate conditions unphosphorylated Pho4 binds to its import receptor,  Pse1, and is translocated into the nucleus.	bind
2385	1	1649	6	10	NULL	0	NULL	Pho4	GP	unphosphorylated	bind					Pse1	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_15_0_291_s_120	10611964	( c) In low-phosphate conditions unphosphorylated Pho4 binds to its import receptor,  Pse1, and is translocated into the nucleus.	bind
2386	2	1649	6	10	NULL	0	NULL	statement 1	Process		occurs in					low-phosphate conditions	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_15_0_291_s_120	10611964	( c) In low-phosphate conditions unphosphorylated Pho4 binds to its import receptor,  Pse1, and is translocated into the nucleus.	bind
2387	3	1649	6	10	NULL	0	NULL	Pho4	GP	unphosphorylated	is translocated to					nucleus	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_15_0_291_s_120	10611964	( c) In low-phosphate conditions unphosphorylated Pho4 binds to its import receptor,  Pse1, and is translocated into the nucleus.	bind
2388	4	1649	6	10	NULL	0	NULL	statement 1	Process		leads to					Statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_15_0_291_s_120	10611964	( c) In low-phosphate conditions unphosphorylated Pho4 binds to its import receptor,  Pse1, and is translocated into the nucleus.	bind
52625	5	1649	6	10	NULL	0	NULL	Pse1	GP		is a type of					import receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_15_0_291_s_120	10611964	( c) In low-phosphate conditions unphosphorylated Pho4 binds to its import receptor,  Pse1, and is translocated into the nucleus.	bind
386	1	1650	5	10	NULL	0	NULL	RecBCD	GP		bind					DNA	NucleicAcid			double-strand tail	NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_15_8181_s_132	11459951	( C) In recombination proficient strains, RecBCD binds to the double-strand tail ( C1); degradation takes place until the first recognized CHI site (CHI is an octameric sequence that switches RecBCD from an exonuclease to a recombinase enzyme) and is followed by a genetic exchange mediated by RecA ( C2); RuvC resolves the first Holliday junction bound by RuvAB ( C3).	bind
387	2	1650	5	10	NULL	0	NULL	RuvAB	GP		bind					Holliday junction	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_15_8181_s_132	11459951	( C) In recombination proficient strains, RecBCD binds to the double-strand tail ( C1); degradation takes place until the first recognized CHI site (CHI is an octameric sequence that switches RecBCD from an exonuclease to a recombinase enzyme) and is followed by a genetic exchange mediated by RecA ( C2); RuvC resolves the first Holliday junction bound by RuvAB ( C3).	bind
388	3	1650	5	10	NULL	0	NULL	RuvC	GP		resolves					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_15_8181_s_132	11459951	( C) In recombination proficient strains, RecBCD binds to the double-strand tail ( C1); degradation takes place until the first recognized CHI site (CHI is an octameric sequence that switches RecBCD from an exonuclease to a recombinase enzyme) and is followed by a genetic exchange mediated by RecA ( C2); RuvC resolves the first Holliday junction bound by RuvAB ( C3).	bind
46159	4	1650	5	10	NULL	0	NULL	RecA	GP		mediate					genetic exchange	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_15_8181_s_132	11459951	( C) In recombination proficient strains, RecBCD binds to the double-strand tail ( C1); degradation takes place until the first recognized CHI site (CHI is an octameric sequence that switches RecBCD from an exonuclease to a recombinase enzyme) and is followed by a genetic exchange mediated by RecA ( C2); RuvC resolves the first Holliday junction bound by RuvAB ( C3).	bind
46161	5	1650	5	10	NULL	0	NULL	RecBCD exonuclease	GP		switches to					RecBCD recombinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_15_8181_s_132	11459951	( C) In recombination proficient strains, RecBCD binds to the double-strand tail ( C1); degradation takes place until the first recognized CHI site (CHI is an octameric sequence that switches RecBCD from an exonuclease to a recombinase enzyme) and is followed by a genetic exchange mediated by RecA ( C2); RuvC resolves the first Holliday junction bound by RuvAB ( C3).	bind
46163	6	1650	5	10	NULL	0	NULL				leads to				CHI site	statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_15_8181_s_132	11459951	( C) In recombination proficient strains, RecBCD binds to the double-strand tail ( C1); degradation takes place until the first recognized CHI site (CHI is an octameric sequence that switches RecBCD from an exonuclease to a recombinase enzyme) and is followed by a genetic exchange mediated by RecA ( C2); RuvC resolves the first Holliday junction bound by RuvAB ( C3).	bind
2480	1	1650	6	10	NULL	0	NULL	RecBCD	GP		bind to					DNA	NucleicAcid			double-strand tail	NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_15_8181_s_132	11459951	( C) In recombination proficient strains, RecBCD binds to the double-strand tail ( C1); degradation takes place until the first recognized CHI site (CHI is an octameric sequence that switches RecBCD from an exonuclease to a recombinase enzyme) and is followed by a genetic exchange mediated by RecA ( C2); RuvC resolves the first Holliday junction bound by RuvAB ( C3).	bind
2481	2	1650	6	10	NULL	0	NULL	RecA	GP		mediates					genetic exchange	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_15_8181_s_132	11459951	( C) In recombination proficient strains, RecBCD binds to the double-strand tail ( C1); degradation takes place until the first recognized CHI site (CHI is an octameric sequence that switches RecBCD from an exonuclease to a recombinase enzyme) and is followed by a genetic exchange mediated by RecA ( C2); RuvC resolves the first Holliday junction bound by RuvAB ( C3).	bind
2482	3	1650	6	10	NULL	0	NULL	RuvAB	GP		bind					Holliday junction	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_15_8181_s_132	11459951	( C) In recombination proficient strains, RecBCD binds to the double-strand tail ( C1); degradation takes place until the first recognized CHI site (CHI is an octameric sequence that switches RecBCD from an exonuclease to a recombinase enzyme) and is followed by a genetic exchange mediated by RecA ( C2); RuvC resolves the first Holliday junction bound by RuvAB ( C3).	bind
2483	4	1650	6	10	NULL	0	NULL	RuvC	GP		resolves					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_15_8181_s_132	11459951	( C) In recombination proficient strains, RecBCD binds to the double-strand tail ( C1); degradation takes place until the first recognized CHI site (CHI is an octameric sequence that switches RecBCD from an exonuclease to a recombinase enzyme) and is followed by a genetic exchange mediated by RecA ( C2); RuvC resolves the first Holliday junction bound by RuvAB ( C3).	bind
2484	5	1650	6	10	NULL	0	NULL	RecBCD exonuclease	GP		switches to 					RecBCD recombinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_15_8181_s_132	11459951	( C) In recombination proficient strains, RecBCD binds to the double-strand tail ( C1); degradation takes place until the first recognized CHI site (CHI is an octameric sequence that switches RecBCD from an exonuclease to a recombinase enzyme) and is followed by a genetic exchange mediated by RecA ( C2); RuvC resolves the first Holliday junction bound by RuvAB ( C3).	bind
2485	6	1650	6	10	NULL	0	NULL				leads to				CH1 site	statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_15_8181_s_132	11459951	( C) In recombination proficient strains, RecBCD binds to the double-strand tail ( C1); degradation takes place until the first recognized CHI site (CHI is an octameric sequence that switches RecBCD from an exonuclease to a recombinase enzyme) and is followed by a genetic exchange mediated by RecA ( C2); RuvC resolves the first Holliday junction bound by RuvAB ( C3).	bind
389	1	1651	5	10	NULL	0	NULL	WASP	GP		bind					proteins	GP		SH3 domain		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jclininvest_111_9_1389_s_184	12727931	( c) In vitro binding of WASP to SH3 domain-containing proteins.	bind
2389	1	1651	6	10	NULL	0	NULL	WASP	GP		bind					protein	GP		SH3 domain containing		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jclininvest_111_9_1389_s_184	12727931	( c) In vitro binding of WASP to SH3 domain-containing proteins.	bind
390	1	1652	5	10	NULL	0	NULL			mutant	does not bind			PH domain		PI(4,5)P2	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_24_13964_s_163	14612561	( C) Incorporation of GFP-actin by Triton cytoskeletons from cells transfected with a  mutant PH domain that does not bind PI(4,5)P2 ( Upper) or by cytoskeletons from cells transfected with PH-GFP, which does bind PI(4,5)P2  ( Lower).	bind
391	2	1652	5	10	NULL	0	NULL				bind			PH-GFP		PI(4,5)P2	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_24_13964_s_163	14612561	( C) Incorporation of GFP-actin by Triton cytoskeletons from cells transfected with a  mutant PH domain that does not bind PI(4,5)P2 ( Upper) or by cytoskeletons from cells transfected with PH-GFP, which does bind PI(4,5)P2  ( Lower).	bind
2486	1	1652	6	10	NULL	0	NULL				bind			PH-GFP		PI(4,5)P2	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_24_13964_s_163	14612561	( C) Incorporation of GFP-actin by Triton cytoskeletons from cells transfected with a  mutant PH domain that does not bind PI(4,5)P2 ( Upper) or by cytoskeletons from cells transfected with PH-GFP, which does bind PI(4,5)P2  ( Lower).	bind
2487	2	1652	6	10	NULL	0	NULL			mutant	does not bind			PH domain		PI(4,5)P2	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_24_13964_s_163	14612561	( C) Incorporation of GFP-actin by Triton cytoskeletons from cells transfected with a  mutant PH domain that does not bind PI(4,5)P2 ( Upper) or by cytoskeletons from cells transfected with PH-GFP, which does bind PI(4,5)P2  ( Lower).	bind
392	1	1653	5	10	NULL	0	NULL	DNA	NucleicAcid		bind					HSF3	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_277_5323_246_s_77	9211854	( C) Induction of HSF3 DNA binding activity by c-Myb.	bind
3163	2	1653	5	10	NULL	0	NULL	statement 1	Process		induce					c-Myb	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_277_5323_246_s_77	9211854	( C) Induction of HSF3 DNA binding activity by c-Myb.	bind
2390	1	1653	6	10	NULL	0	NULL	HSF3	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_science_277_5323_246_s_77	9211854	( C) Induction of HSF3 DNA binding activity by c-Myb.	bind
2391	2	1653	6	10	NULL	0	NULL	c-Myb	GP		induces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_277_5323_246_s_77	9211854	( C) Induction of HSF3 DNA binding activity by c-Myb.	bind
393	1	1654	5	10	NULL	0	NULL	importin-beta	GP		bind					NuMA	GP	endogenous			NULL		NULL	NULL	NULL	NULL	gw60_science_291_5504_653_s_96	11229403	( C) Inhibition of binding of importin-beta to endogenous NuMA by RanL43E.	bind
395	2	1654	5	10	NULL	0	NULL	Ran	GP		inhibit			L43E		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_291_5504_653_s_96	11229403	( C) Inhibition of binding of importin-beta to endogenous NuMA by RanL43E.	bind
2392	1	1654	6	10	NULL	0	NULL	importin-beta	GP		bind					NuMA	GP	endogenous			NULL		NULL	NULL	NULL	NULL	gw60_science_291_5504_653_s_96	11229403	( C) Inhibition of binding of importin-beta to endogenous NuMA by RanL43E.	bind
2393	2	1654	6	10	NULL	0	NULL	Ran	GP		inhibits			L43E		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_291_5504_653_s_96	11229403	( C) Inhibition of binding of importin-beta to endogenous NuMA by RanL43E.	bind
396	1	1655	5	10	NULL	0	NULL	PIP2	Chemical		bind					GFP-PHD	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5419_1527_s_35	10348740	( C) Inhibition of PIP2 binding of 2 muM GFP-PHD by 2 muM IP3 (InsP3), inositol 1,3,4-trisphosphate [Ins(1,3,4)P3], and inositol 1,3,4,5-tetrakisphosphate (InsP4).	bind
397	2	1655	5	10	NULL	0	NULL	InsP3	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5419_1527_s_35	10348740	( C) Inhibition of PIP2 binding of 2 muM GFP-PHD by 2 muM IP3 (InsP3), inositol 1,3,4-trisphosphate [Ins(1,3,4)P3], and inositol 1,3,4,5-tetrakisphosphate (InsP4).	bind
398	3	1655	5	10	NULL	0	NULL	InsP3	Chemical		is					IP3	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5419_1527_s_35	10348740	( C) Inhibition of PIP2 binding of 2 muM GFP-PHD by 2 muM IP3 (InsP3), inositol 1,3,4-trisphosphate [Ins(1,3,4)P3], and inositol 1,3,4,5-tetrakisphosphate (InsP4).	bind
400	4	1655	5	10	NULL	0	NULL	Ins(1,3,4)P3	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5419_1527_s_35	10348740	( C) Inhibition of PIP2 binding of 2 muM GFP-PHD by 2 muM IP3 (InsP3), inositol 1,3,4-trisphosphate [Ins(1,3,4)P3], and inositol 1,3,4,5-tetrakisphosphate (InsP4).	bind
401	5	1655	5	10	NULL	0	NULL	Ins(1,3,4)P3	Chemical		is					inositol 1,3,4-trisphosphate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5419_1527_s_35	10348740	( C) Inhibition of PIP2 binding of 2 muM GFP-PHD by 2 muM IP3 (InsP3), inositol 1,3,4-trisphosphate [Ins(1,3,4)P3], and inositol 1,3,4,5-tetrakisphosphate (InsP4).	bind
402	6	1655	5	10	NULL	0	NULL	InsP4	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5419_1527_s_35	10348740	( C) Inhibition of PIP2 binding of 2 muM GFP-PHD by 2 muM IP3 (InsP3), inositol 1,3,4-trisphosphate [Ins(1,3,4)P3], and inositol 1,3,4,5-tetrakisphosphate (InsP4).	bind
403	7	1655	5	10	NULL	0	NULL	InsP4	Chemical		is					inositol 1,3,4,5-tetrakisphosphate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5419_1527_s_35	10348740	( C) Inhibition of PIP2 binding of 2 muM GFP-PHD by 2 muM IP3 (InsP3), inositol 1,3,4-trisphosphate [Ins(1,3,4)P3], and inositol 1,3,4,5-tetrakisphosphate (InsP4).	bind
2394	1	1655	6	10	NULL	0	NULL	PIP2	Chemical		bind					GFP-PHD	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5419_1527_s_35	10348740	( C) Inhibition of PIP2 binding of 2 muM GFP-PHD by 2 muM IP3 (InsP3), inositol 1,3,4-trisphosphate [Ins(1,3,4)P3], and inositol 1,3,4,5-tetrakisphosphate (InsP4).	bind
2395	2	1655	6	10	NULL	0	NULL	IP3	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5419_1527_s_35	10348740	( C) Inhibition of PIP2 binding of 2 muM GFP-PHD by 2 muM IP3 (InsP3), inositol 1,3,4-trisphosphate [Ins(1,3,4)P3], and inositol 1,3,4,5-tetrakisphosphate (InsP4).	bind
2396	3	1655	6	10	NULL	0	NULL	Ins(1,3,4)P3	Chemical		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5419_1527_s_35	10348740	( C) Inhibition of PIP2 binding of 2 muM GFP-PHD by 2 muM IP3 (InsP3), inositol 1,3,4-trisphosphate [Ins(1,3,4)P3], and inositol 1,3,4,5-tetrakisphosphate (InsP4).	bind
2397	4	1655	6	10	NULL	0	NULL	Ins(1,3,4)P3	Chemical		is					inositol 1,3,4-trisphosphate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5419_1527_s_35	10348740	( C) Inhibition of PIP2 binding of 2 muM GFP-PHD by 2 muM IP3 (InsP3), inositol 1,3,4-trisphosphate [Ins(1,3,4)P3], and inositol 1,3,4,5-tetrakisphosphate (InsP4).	bind
2398	5	1655	6	10	NULL	0	NULL	InsP4	Chemical		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5419_1527_s_35	10348740	( C) Inhibition of PIP2 binding of 2 muM GFP-PHD by 2 muM IP3 (InsP3), inositol 1,3,4-trisphosphate [Ins(1,3,4)P3], and inositol 1,3,4,5-tetrakisphosphate (InsP4).	bind
2399	6	1655	6	10	NULL	0	NULL	InsP4	Chemical		is					inositol 1,3,4,5-tetrakisphosphate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5419_1527_s_35	10348740	( C) Inhibition of PIP2 binding of 2 muM GFP-PHD by 2 muM IP3 (InsP3), inositol 1,3,4-trisphosphate [Ins(1,3,4)P3], and inositol 1,3,4,5-tetrakisphosphate (InsP4).	bind
3077	7	1655	6	10	NULL	0	NULL	IP3	Chemical		is					InsP3	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5419_1527_s_35	10348740	( C) Inhibition of PIP2 binding of 2 muM GFP-PHD by 2 muM IP3 (InsP3), inositol 1,3,4-trisphosphate [Ins(1,3,4)P3], and inositol 1,3,4,5-tetrakisphosphate (InsP4).	bind
405	1	1656	5	10	NULL	0	NULL	biotin-HKa	GP		bind					tropomyosin	GP	purified			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_19_12224_s_158	12196635	( C) Inhibition of the binding of biotin-HKa (10 nM) to purified tropomyosin by HKa D5.	bind
406	2	1656	5	10	NULL	0	NULL	HKa D5	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_19_12224_s_158	12196635	( C) Inhibition of the binding of biotin-HKa (10 nM) to purified tropomyosin by HKa D5.	bind
2400	1	1656	6	10	NULL	0	NULL	biotin-HKa	GP		bind					tropomyosin	GP	purified			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_19_12224_s_158	12196635	( C) Inhibition of the binding of biotin-HKa (10 nM) to purified tropomyosin by HKa D5.	bind
2401	2	1656	6	10	NULL	0	NULL	HKaD5	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_19_12224_s_158	12196635	( C) Inhibition of the binding of biotin-HKa (10 nM) to purified tropomyosin by HKa D5.	bind
899	2	1657	5	10	NULL	0	NULL	HoxD9	GP	2H,15N-labeled 	bind			 homeodomain		Nhb nonspecific DNA duplexes 	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_41_15062_s_44	17008406	( c) Intermolecular 1HN-gamma2 PREs arising from the dT-EDTA-Mn2+ measured on uniformly 2H,15N-labeled HoxD9 homeodomain bound to the Nhb nonspecific ( Left) and Shb-specific ( Right) DNA duplexes at 20 mM NaCl.	bind
900	3	1657	5	10	NULL	0	NULL	HoxD9	GP	2H,15N-labeled 	bind			 homeodomain		Shb-specific DNA duplexes 	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_41_15062_s_44	17008406	( c) Intermolecular 1HN-gamma2 PREs arising from the dT-EDTA-Mn2+ measured on uniformly 2H,15N-labeled HoxD9 homeodomain bound to the Nhb nonspecific ( Left) and Shb-specific ( Right) DNA duplexes at 20 mM NaCl.	bind
2488	1	1657	6	10	NULL	0	NULL	HoxD9	GP	2H,15N-labeled	bind			homeodomain		Nhb nonspecific DNA duplexes	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_41_15062_s_44	17008406	( c) Intermolecular 1HN-gamma2 PREs arising from the dT-EDTA-Mn2+ measured on uniformly 2H,15N-labeled HoxD9 homeodomain bound to the Nhb nonspecific ( Left) and Shb-specific ( Right) DNA duplexes at 20 mM NaCl.	bind
2489	2	1657	6	10	NULL	0	NULL	HoxD9	GP	2H,15N-labeled	bind			homeodomain		Shb-specific DNA duplexes	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_41_15062_s_44	17008406	( c) Intermolecular 1HN-gamma2 PREs arising from the dT-EDTA-Mn2+ measured on uniformly 2H,15N-labeled HoxD9 homeodomain bound to the Nhb nonspecific ( Left) and Shb-specific ( Right) DNA duplexes at 20 mM NaCl.	bind
408	1	1659	5	10	NULL	0	NULL	vinculin 	GP		bind					F-actin	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_5853_s_179	10545097	( C) IpaA induces vinculin binding to immobilized F-actin.	bind
409	2	1659	5	10	NULL	0	NULL	IpaA	GP		induces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_5853_s_179	10545097	( C) IpaA induces vinculin binding to immobilized F-actin.	bind
2492	1	1659	6	10	NULL	0	NULL	vinculin	GP		bind					F-actin	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_5853_s_179	10545097	( C) IpaA induces vinculin binding to immobilized F-actin.	bind
2493	2	1659	6	10	NULL	0	NULL	IpaA	GP		induces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_5853_s_179	10545097	( C) IpaA induces vinculin binding to immobilized F-actin.	bind
410	1	1660	5	10	NULL	0	NULL	talin	GP		bind					vinculin	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_5853_s_85	10545097	( C) IpaA inhibits talin binding to vinculin.	bind
411	2	1660	5	10	NULL	0	NULL	IpaA	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_5853_s_85	10545097	( C) IpaA inhibits talin binding to vinculin.	bind
2495	1	1660	6	10	NULL	0	NULL	talin	GP		bind					vinculin	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_5853_s_85	10545097	( C) IpaA inhibits talin binding to vinculin.	bind
2496	2	1660	6	10	NULL	0	NULL	IpaA	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_5853_s_85	10545097	( C) IpaA inhibits talin binding to vinculin.	bind
412	1	1661	5	10	NULL	0	NULL	p31comet	GP		bind					N2-Mad2	GP		R133A		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_15_3133_s_137	15257285	( C) ITC analysis of the binding between p31comet and N2-Mad2R133A.	bind
2497	1	1661	6	10	NULL	0	NULL	p31comet	GP		bind					N2-Mad2	GP		R133A		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_15_3133_s_137	15257285	( C) ITC analysis of the binding between p31comet and N2-Mad2R133A.	bind
413	1	1662	5	10	NULL	0	NULL	JNKK1	GP		bind					JNK1	GP	endogenous			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_21_3369_s_201	9808624	( C) JNKK1 binds endogenous JNK1.	bind
2498	1	1662	6	10	NULL	0	NULL	JNKK1	GP		bind					JNK1	GP	endogenous			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_21_3369_s_201	9808624	( C) JNKK1 binds endogenous JNK1.	bind
414	1	1663	5	10	NULL	0	NULL	P15 INK4b	GP		bind					Cdk4	GP				NULL	MEFs treated with TGF-beta	NULL	NULL	NULL	NULL	gw60_embo_19_13_3496_s_120	10880462	( C) Levels of P15 INK4b, P16 INK4a, P21 Cip1 and P27 Kip1 proteins bound to Cdk4 in MEFs treated with TGF-beta for the times indicated.	bind
415	2	1663	5	10	NULL	0	NULL	P16 INK4a	GP		bind					Cdk4	GP				NULL	MEFs treated with TGF-beta	NULL	NULL	NULL	NULL	gw60_embo_19_13_3496_s_120	10880462	( C) Levels of P15 INK4b, P16 INK4a, P21 Cip1 and P27 Kip1 proteins bound to Cdk4 in MEFs treated with TGF-beta for the times indicated.	bind
416	3	1663	5	10	NULL	0	NULL	P21 Cip1	GP		bind					Cdk4	GP				NULL	MEFs treated with TGF-beta	NULL	NULL	NULL	NULL	gw60_embo_19_13_3496_s_120	10880462	( C) Levels of P15 INK4b, P16 INK4a, P21 Cip1 and P27 Kip1 proteins bound to Cdk4 in MEFs treated with TGF-beta for the times indicated.	bind
417	4	1663	5	10	NULL	0	NULL	P27 Kip1	GP		bind					Cdk4	GP				NULL	MEFs treated with TGF-beta	NULL	NULL	NULL	NULL	gw60_embo_19_13_3496_s_120	10880462	( C) Levels of P15 INK4b, P16 INK4a, P21 Cip1 and P27 Kip1 proteins bound to Cdk4 in MEFs treated with TGF-beta for the times indicated.	bind
2499	1	1663	6	10	NULL	0	NULL	P15 INK4b	GP		bind					Cdk4	GP				NULL	MEFs treated with TGF-beta	NULL	NULL	NULL	NULL	gw60_embo_19_13_3496_s_120	10880462	( C) Levels of P15 INK4b, P16 INK4a, P21 Cip1 and P27 Kip1 proteins bound to Cdk4 in MEFs treated with TGF-beta for the times indicated.	bind
2500	2	1663	6	10	NULL	0	NULL	P16 INK4a	GP		bind					Cdk4	GP				NULL	MEFs treated with TGF-beta	NULL	NULL	NULL	NULL	gw60_embo_19_13_3496_s_120	10880462	( C) Levels of P15 INK4b, P16 INK4a, P21 Cip1 and P27 Kip1 proteins bound to Cdk4 in MEFs treated with TGF-beta for the times indicated.	bind
2501	3	1663	6	10	NULL	0	NULL	P21 Cip1	GP		bind					Cdk4	GP				NULL	MEFs treated with TGF-beta	NULL	NULL	NULL	NULL	gw60_embo_19_13_3496_s_120	10880462	( C) Levels of P15 INK4b, P16 INK4a, P21 Cip1 and P27 Kip1 proteins bound to Cdk4 in MEFs treated with TGF-beta for the times indicated.	bind
2502	4	1663	6	10	NULL	0	NULL	P27 Kip1	GP		bind					Cdk4	GP				NULL	MEFs treated with TGF-beta	NULL	NULL	NULL	NULL	gw60_embo_19_13_3496_s_120	10880462	( C) Levels of P15 INK4b, P16 INK4a, P21 Cip1 and P27 Kip1 proteins bound to Cdk4 in MEFs treated with TGF-beta for the times indicated.	bind
2539	1	1664	6	10	NULL	0	NULL	HP1beta	GP	GFP full length	bind 					 histone H3	GP	methylated	W42L;;Lys-9		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_489_s_156	14765118	( C) Localisation of GFP full-length HP1beta with point mutations that cripple binding to Lys-9-methylated histone H3 (W42L),  Lys-9-methylated histone H3 and PXVXL proteins (W42L, W170), dimerisation and binding  to PXVXL proteins (I161E), and dimerisation and binding to PXVXL proteins and binding  to Lys-9-methylated histone H3 (W42L, I161E).	bind
2540	2	1664	6	10	NULL	0	NULL	HP1beta	GP	mutant;;GFP full length	cripple					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_489_s_156	14765118	( C) Localisation of GFP full-length HP1beta with point mutations that cripple binding to Lys-9-methylated histone H3 (W42L),  Lys-9-methylated histone H3 and PXVXL proteins (W42L, W170), dimerisation and binding  to PXVXL proteins (I161E), and dimerisation and binding to PXVXL proteins and binding  to Lys-9-methylated histone H3 (W42L, I161E).	bind
2541	3	1664	6	10	NULL	0	NULL	HP1beta	GP	GFP full length	bind					PXVXL proteins	GP		W42L;;W170		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_489_s_156	14765118	( C) Localisation of GFP full-length HP1beta with point mutations that cripple binding to Lys-9-methylated histone H3 (W42L),  Lys-9-methylated histone H3 and PXVXL proteins (W42L, W170), dimerisation and binding  to PXVXL proteins (I161E), and dimerisation and binding to PXVXL proteins and binding  to Lys-9-methylated histone H3 (W42L, I161E).	bind
2542	4	1664	6	10	NULL	0	NULL	HP1beta	GP	mutant;;GFP full length	cripple					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_489_s_156	14765118	( C) Localisation of GFP full-length HP1beta with point mutations that cripple binding to Lys-9-methylated histone H3 (W42L),  Lys-9-methylated histone H3 and PXVXL proteins (W42L, W170), dimerisation and binding  to PXVXL proteins (I161E), and dimerisation and binding to PXVXL proteins and binding  to Lys-9-methylated histone H3 (W42L, I161E).	bind
3080	5	1664	6	10	NULL	0	NULL	HP1 beta	GP	GFP full length	bind					PXVXL protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_489_s_156	14765118	( C) Localisation of GFP full-length HP1beta with point mutations that cripple binding to Lys-9-methylated histone H3 (W42L),  Lys-9-methylated histone H3 and PXVXL proteins (W42L, W170), dimerisation and binding  to PXVXL proteins (I161E), and dimerisation and binding to PXVXL proteins and binding  to Lys-9-methylated histone H3 (W42L, I161E).	bind
4025	6	1664	6	10	NULL	0	NULL	HP1 beta	GP	mutant;;GFP full length	cripple					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_489_s_156	14765118	( C) Localisation of GFP full-length HP1beta with point mutations that cripple binding to Lys-9-methylated histone H3 (W42L),  Lys-9-methylated histone H3 and PXVXL proteins (W42L, W170), dimerisation and binding  to PXVXL proteins (I161E), and dimerisation and binding to PXVXL proteins and binding  to Lys-9-methylated histone H3 (W42L, I161E).	bind
4026	7	1664	6	10	NULL	0	NULL	HP1 beta	GP	GFP full length	bind					PXVXL protein	GP		I161E		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_489_s_156	14765118	( C) Localisation of GFP full-length HP1beta with point mutations that cripple binding to Lys-9-methylated histone H3 (W42L),  Lys-9-methylated histone H3 and PXVXL proteins (W42L, W170), dimerisation and binding  to PXVXL proteins (I161E), and dimerisation and binding to PXVXL proteins and binding  to Lys-9-methylated histone H3 (W42L, I161E).	bind
4027	8	1664	6	10	NULL	0	NULL	HP1 beta	GP	mutant;;GFP full length	cripple					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_489_s_156	14765118	( C) Localisation of GFP full-length HP1beta with point mutations that cripple binding to Lys-9-methylated histone H3 (W42L),  Lys-9-methylated histone H3 and PXVXL proteins (W42L, W170), dimerisation and binding  to PXVXL proteins (I161E), and dimerisation and binding to PXVXL proteins and binding  to Lys-9-methylated histone H3 (W42L, I161E).	bind
4028	9	1664	6	10	NULL	0	NULL	HP1 beta	GP	mutant;;GFP full length	cripple					PXVXL protein	GP	dimerisation of	I161E		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_489_s_156	14765118	( C) Localisation of GFP full-length HP1beta with point mutations that cripple binding to Lys-9-methylated histone H3 (W42L),  Lys-9-methylated histone H3 and PXVXL proteins (W42L, W170), dimerisation and binding  to PXVXL proteins (I161E), and dimerisation and binding to PXVXL proteins and binding  to Lys-9-methylated histone H3 (W42L, I161E).	bind
52805	10	1664	6	10	NULL	0	NULL	HP1beta	GP	GFP full length	bind					histone H3	GP	methylated	Lys-9		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_489_s_156	14765118	( C) Localisation of GFP full-length HP1beta with point mutations that cripple binding to Lys-9-methylated histone H3 (W42L),  Lys-9-methylated histone H3 and PXVXL proteins (W42L, W170), dimerisation and binding  to PXVXL proteins (I161E), and dimerisation and binding to PXVXL proteins and binding  to Lys-9-methylated histone H3 (W42L, I161E).	bind
52806	11	1664	6	10	NULL	0	NULL	HP1beta	GP	mutant;;GFP full length	cripple					statement 10	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_489_s_156	14765118	( C) Localisation of GFP full-length HP1beta with point mutations that cripple binding to Lys-9-methylated histone H3 (W42L),  Lys-9-methylated histone H3 and PXVXL proteins (W42L, W170), dimerisation and binding  to PXVXL proteins (I161E), and dimerisation and binding to PXVXL proteins and binding  to Lys-9-methylated histone H3 (W42L, I161E).	bind
52808	12	1664	6	10	NULL	0	NULL	HP1beta	GP	mutant;;GFP full length	cripple					PXVXL proteins	GP	dimerisation of			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_489_s_156	14765118	( C) Localisation of GFP full-length HP1beta with point mutations that cripple binding to Lys-9-methylated histone H3 (W42L),  Lys-9-methylated histone H3 and PXVXL proteins (W42L, W170), dimerisation and binding  to PXVXL proteins (I161E), and dimerisation and binding to PXVXL proteins and binding  to Lys-9-methylated histone H3 (W42L, I161E).	bind
52809	13	1664	6	10	NULL	0	NULL	HP1beta	GP	GFP full length	bind					histone H3	GP	methylated	W42L;; I161E;;Lys-9		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_489_s_156	14765118	( C) Localisation of GFP full-length HP1beta with point mutations that cripple binding to Lys-9-methylated histone H3 (W42L),  Lys-9-methylated histone H3 and PXVXL proteins (W42L, W170), dimerisation and binding  to PXVXL proteins (I161E), and dimerisation and binding to PXVXL proteins and binding  to Lys-9-methylated histone H3 (W42L, I161E).	bind
52810	14	1664	6	10	NULL	0	NULL	HP1beta	GP	mutant;;GFP full length	cripple					statement 13	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_489_s_156	14765118	( C) Localisation of GFP full-length HP1beta with point mutations that cripple binding to Lys-9-methylated histone H3 (W42L),  Lys-9-methylated histone H3 and PXVXL proteins (W42L, W170), dimerisation and binding  to PXVXL proteins (I161E), and dimerisation and binding to PXVXL proteins and binding  to Lys-9-methylated histone H3 (W42L, I161E).	bind
418	1	1665	5	10	NULL	0	NULL	mAb LM-142	GP		bind					protein A/G resin	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_4_1163_s_92	15657120	( C) mAb LM-142 was bound to protein A/G resin and coated with secreted purified alphavbeta3 (500 ng).	bind
419	2	1665	5	10	NULL	0	NULL	mAb LM-142	GP		coated with					alphavbeta3	GP	secreted;; purified 			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_4_1163_s_92	15657120	( C) mAb LM-142 was bound to protein A/G resin and coated with secreted purified alphavbeta3 (500 ng).	bind
2503	1	1665	6	10	NULL	0	NULL	mAb LM-142	GP		bind					A/G resin protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_4_1163_s_92	15657120	( C) mAb LM-142 was bound to protein A/G resin and coated with secreted purified alphavbeta3 (500 ng).	bind
2504	2	1665	6	10	NULL	0	NULL	mAb LM-142	GP		coated with					alphavbeta3	GP	secreted;;purified			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_4_1163_s_92	15657120	( C) mAb LM-142 was bound to protein A/G resin and coated with secreted purified alphavbeta3 (500 ng).	bind
420	1	1666	5	10	NULL	0	NULL	calmodulin	GP		bind					MLCK	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_5_1159_s_108	16432210	( C) Main-chain ribbon diagrams of calmodulin (yellow) bound to the target proteins myosin  light chain kinase (MLCK), SK channel, GAD, and EF (red).	bind
421	2	1666	5	10	NULL	0	NULL	MLCK	GP		is					myosin light chain kinase	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_5_1159_s_108	16432210	( C) Main-chain ribbon diagrams of calmodulin (yellow) bound to the target proteins myosin  light chain kinase (MLCK), SK channel, GAD, and EF (red).	bind
422	3	1666	5	10	NULL	0	NULL	calmodulin	GP		bind					SK channel	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_5_1159_s_108	16432210	( C) Main-chain ribbon diagrams of calmodulin (yellow) bound to the target proteins myosin  light chain kinase (MLCK), SK channel, GAD, and EF (red).	bind
423	4	1666	5	10	NULL	0	NULL	calmodulin	GP		bind					GAD	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_5_1159_s_108	16432210	( C) Main-chain ribbon diagrams of calmodulin (yellow) bound to the target proteins myosin  light chain kinase (MLCK), SK channel, GAD, and EF (red).	bind
424	5	1666	5	10	NULL	0	NULL	calmodulin	GP		bind					EF	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_5_1159_s_108	16432210	( C) Main-chain ribbon diagrams of calmodulin (yellow) bound to the target proteins myosin  light chain kinase (MLCK), SK channel, GAD, and EF (red).	bind
2505	1	1666	6	10	NULL	0	NULL	calmodulin	GP		bind to					MLCK	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_5_1159_s_108	16432210	( C) Main-chain ribbon diagrams of calmodulin (yellow) bound to the target proteins myosin  light chain kinase (MLCK), SK channel, GAD, and EF (red).	bind
2506	2	1666	6	10	NULL	0	NULL	calmodulin	GP		bind to					SK channel	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_5_1159_s_108	16432210	( C) Main-chain ribbon diagrams of calmodulin (yellow) bound to the target proteins myosin  light chain kinase (MLCK), SK channel, GAD, and EF (red).	bind
2507	3	1666	6	10	NULL	0	NULL	calmodulin	GP		bind to					GAD	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_5_1159_s_108	16432210	( C) Main-chain ribbon diagrams of calmodulin (yellow) bound to the target proteins myosin  light chain kinase (MLCK), SK channel, GAD, and EF (red).	bind
2508	4	1666	6	10	NULL	0	NULL	calmodulin	GP		bind to					EF	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_5_1159_s_108	16432210	( C) Main-chain ribbon diagrams of calmodulin (yellow) bound to the target proteins myosin  light chain kinase (MLCK), SK channel, GAD, and EF (red).	bind
45936	5	1666	6	10	NULL	0	NULL	MLCK	GP		is					myosin light chain kinase	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_5_1159_s_108	16432210	( C) Main-chain ribbon diagrams of calmodulin (yellow) bound to the target proteins myosin  light chain kinase (MLCK), SK channel, GAD, and EF (red).	bind
505	1	1667	5	10	NULL	0	NULL	Mant-GTP	GP		bind					Rac1A	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_7_1620_s_179	11285226	( C) Mant-GTP binding to Rac1A results in an increase in fluorescence.	bind
2509	1	1667	6	10	NULL	0	NULL	Mant-GTP	GP		bind to					Rac1A	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_7_1620_s_179	11285226	( C) Mant-GTP binding to Rac1A results in an increase in fluorescence.	bind
425	1	1668	5	10	NULL	0	NULL	AKIN10	GP		bind					AKIN11	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_9_5322_s_38	10220464	( C) Mapping of PRL1 domain involved in binding of AKIN10 and AKIN11.	bind
426	2	1668	5	10	NULL	0	NULL				involved in			PRL1 domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_9_5322_s_38	10220464	( C) Mapping of PRL1 domain involved in binding of AKIN10 and AKIN11.	bind
2510	1	1668	6	10	NULL	0	NULL	AKIN11	GP		bind					AKIN10	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_9_5322_s_38	10220464	( C) Mapping of PRL1 domain involved in binding of AKIN10 and AKIN11.	bind
2511	2	1668	6	10	NULL	0	NULL				is involved in			PRL1 domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_9_5322_s_38	10220464	( C) Mapping of PRL1 domain involved in binding of AKIN10 and AKIN11.	bind
427	1	1669	5	10	NULL	0	NULL	MBP - Kap114p	GP		bind					GST - histones	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_23_6527_s_103	12456659	( C) MBP - Kap114p (200 nM) binding to GST - histones as in	bind
2512	1	1669	6	10	NULL	0	NULL	MBP - Kap114p	GP		bind					GST - histones	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_23_6527_s_103	12456659	( C) MBP - Kap114p (200 nM) binding to GST - histones as in	bind
428	1	1670	5	10	NULL	0	NULL	P2	GP		bind					CHO cell line	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_105_6_793_s_218	10727448	( c) Mean fluorescence intensity of P2 binding to the 3 CHO cell lines.	bind
2513	1	1670	6	10	NULL	0	NULL	P2	GP		bind					CHO cell lines	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_105_6_793_s_218	10727448	( c) Mean fluorescence intensity of P2 binding to the 3 CHO cell lines.	bind
429	1	1671	5	10	NULL	0	NULL	MED-1	GP		bind					tbx-35	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_development_133_16_3097_s_106	16831832	( C) MED-1 binds the  tbx-35 promoter.	bind
2514	1	1671	6	10	NULL	0	NULL	MED-1	GP		bind					tbx-35	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_development_133_16_3097_s_106	16831832	( C) MED-1 binds the  tbx-35 promoter.	bind
430	1	1672	5	10	NULL	0	NULL	MEF2C 	GP		bind					PGC-1alpha	GP			MEF-binding site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_12_7111_s_112	12764228	( C) MEF2C binds to the MEF-binding site in the  PGC-1alpha promoter.	bind
2515	1	1672	6	10	NULL	0	NULL	MEF2C	GP		bind					PGC-1alpha	GP			MEF binding site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_12_7111_s_112	12764228	( C) MEF2C binds to the MEF-binding site in the  PGC-1alpha promoter.	bind
431	1	1673	5	10	NULL	0	NULL	PS1	GP		bind		preferentially			Nct	GP	mature			NULL	membrane fractions of HEK 293 cells	NULL	NULL	NULL	NULL	gw60_pnas_99_13_8666_s_87	12048259	( C) Membrane fractions of HEK 293 cells stably coexpressing swAPP and Nct were solubilized with CHAPS and analyzed for PS/Nct interactions as in  B. Note that PS1 preferentially binds to mature Nct. ( D) HEK 293 cells stably coexpressing swAPP, wild-type PS1, and wild-type Nct were treated with cycloheximide (100 mug/ml) for the indicated time points.	bind
2516	1	1673	6	10	NULL	0	NULL	PS1	GP		bind		preferentially			Nct	GP	mature			NULL	HEK293 cells treated with cycloheximide	NULL	NULL	NULL	NULL	gw60_pnas_99_13_8666_s_87	12048259	( C) Membrane fractions of HEK 293 cells stably coexpressing swAPP and Nct were solubilized with CHAPS and analyzed for PS/Nct interactions as in  B. Note that PS1 preferentially binds to mature Nct. ( D) HEK 293 cells stably coexpressing swAPP, wild-type PS1, and wild-type Nct were treated with cycloheximide (100 mug/ml) for the indicated time points.	bind
432	1	1674	5	10	NULL	0	NULL	trimeric MBP subunits	GP	dimer of	bind					MASP2	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_10_2348_s_220	12743029	( C) Model of a dimer of trimeric MBP subunits bound to the MASP2 model shown in	bind
2517	1	1674	6	10	NULL	0	NULL	trimeric MBP subunits	GP	dimer of	bind					MASP2	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_10_2348_s_220	12743029	( C) Model of a dimer of trimeric MBP subunits bound to the MASP2 model shown in	bind
433	1	1675	5	10	NULL	0	NULL	TF1-v1	GP		bind					theophylline	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_7_1631_s_150	11266567	( C) Model of TF1-v1 bound to theophylline (encircled T).	bind
2518	1	1675	6	10	NULL	0	NULL	TF1-v1	GP		bind					theophylline	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_7_1631_s_150	11266567	( C) Model of TF1-v1 bound to theophylline (encircled T).	bind
434	1	1676	5	10	NULL	0	NULL	SUMO1	GP		modify					SATB2	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_24_3048_s_117	14701874	( C) Modification of SATB2 by SUMO1 and SUMO3.	bind
435	2	1676	5	10	NULL	0	NULL	SUMO3	GP		modify					SATB2	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_24_3048_s_117	14701874	( C) Modification of SATB2 by SUMO1 and SUMO3.	bind
2519	1	1676	6	10	NULL	0	NULL	SUMO1	GP		modify					SATB2	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_24_3048_s_117	14701874	( C) Modification of SATB2 by SUMO1 and SUMO3.	bind
2520	2	1676	6	10	NULL	0	NULL	SUMO3	GP		modify					SATB2	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_24_3048_s_117	14701874	( C) Modification of SATB2 by SUMO1 and SUMO3.	bind
436	1	1677	5	10	NULL	0	NULL	GST-Src	GP		bind			 SH2		PSD-95 peptides	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_20_4971_s_206	16990796	( C) Modified ELISAs to measure binding of GST-Src SH2 to each of the PSD-95 peptides.	bind
2521	1	1677	6	10	NULL	0	NULL	GST-Src	GP		bind			SH2		PSD-95 peptides	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_20_4971_s_206	16990796	( C) Modified ELISAs to measure binding of GST-Src SH2 to each of the PSD-95 peptides.	bind
437	1	1678	5	10	NULL	0	NULL	Mre11p	GP		bind					telomere	Chromosome				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_19_10854_s_161	12963812	( c) Mre11p and Xrs2p binding to telomeres.	bind
438	2	1678	5	10	NULL	0	NULL	Xrs2p	GP		bind					telomere	Chromosome				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_19_10854_s_161	12963812	( c) Mre11p and Xrs2p binding to telomeres.	bind
2522	1	1678	6	10	NULL	0	NULL	Mre11p	GP		bind					telomere	Chromosome				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_19_10854_s_161	12963812	( c) Mre11p and Xrs2p binding to telomeres.	bind
2523	2	1678	6	10	NULL	0	NULL	Xrs2p	GP		bind					telomere	Chromosome				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_19_10854_s_161	12963812	( c) Mre11p and Xrs2p binding to telomeres.	bind
439	1	1679	5	10	NULL	0	NULL	MT	CellComponent		bind					KIF1A	GP	deletion variants			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1506_s_72	15014437	( C) MT binding of the KIF1A deletion variants.	bind
2524	1	1679	6	10	NULL	0	NULL	KIF1A	GP	deletion variants	bind					MT	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1506_s_72	15014437	( C) MT binding of the KIF1A deletion variants.	bind
440	1	1680	5	10	NULL	0	NULL	MT	CellComponent		bind					KIF1A	GP	deletions			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1506_s_42	15014437	( C) MT-binding properties of the KIF1A deletions.	bind
2525	1	1680	6	10	NULL	0	NULL	KIF1A	GP	deletions	bind					MT	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1506_s_42	15014437	( C) MT-binding properties of the KIF1A deletions.	bind
441	1	1681	5	10	NULL	0	NULL	PpPex7p	GP	mutated	does not bind					ScFox3p	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_140_4_807_s_375	9472033	( C) Mutated PpPex7p fails to bind to ScFox3p  in a two-hybrid analysis.	bind
2526	1	1681	6	10	NULL	0	NULL	PpPex7p	GP	mutant	does not bind					ScFox3p	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_140_4_807_s_375	9472033	( C) Mutated PpPex7p fails to bind to ScFox3p  in a two-hybrid analysis.	bind
442	1	1683	5	10	NULL	0	NULL	ZF5	GP		bind									RRS	NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_26_14991_s_141	11734633	( C) Mutations in zinc fingers 3 and 4 disrupt binding of ZF5 to the RRS.	bind
443	2	1683	5	10	NULL	0	NULL	ZF5	GP		disrupt			mutant zinc finger 3		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_26_14991_s_141	11734633	( C) Mutations in zinc fingers 3 and 4 disrupt binding of ZF5 to the RRS.	bind
444	3	1683	5	10	NULL	0	NULL	ZF5	GP		disrupt			mutant zinc finger 4		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_26_14991_s_141	11734633	( C) Mutations in zinc fingers 3 and 4 disrupt binding of ZF5 to the RRS.	bind
2527	1	1683	6	10	NULL	0	NULL	ZF5	GP		bind									RRS	NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_26_14991_s_141	11734633	( C) Mutations in zinc fingers 3 and 4 disrupt binding of ZF5 to the RRS.	bind
2528	2	1683	6	10	NULL	0	NULL	ZF5	GP		disrupt			mutant zinc finger 3		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_26_14991_s_141	11734633	( C) Mutations in zinc fingers 3 and 4 disrupt binding of ZF5 to the RRS.	bind
2529	3	1683	6	10	NULL	0	NULL	ZF5	GP		disrupt			mutant zinc finger 4		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_26_14991_s_141	11734633	( C) Mutations in zinc fingers 3 and 4 disrupt binding of ZF5 to the RRS.	bind
445	1	1684	5	10	NULL	0	NULL	SIP1	GP		bind			FS		alpha4I	GP	WT			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5073_s_199	10487759	( C) Mutations within NZF3, NZF4, CZF2 or CZF3 abolish the binding of SIP1FS to alpha4IWT.	bind
446	2	1684	5	10	NULL	0	NULL			mutant	abolish			NZF3		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5073_s_199	10487759	( C) Mutations within NZF3, NZF4, CZF2 or CZF3 abolish the binding of SIP1FS to alpha4IWT.	bind
447	3	1684	5	10	NULL	0	NULL			mutant	abolish			NZF4		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5073_s_199	10487759	( C) Mutations within NZF3, NZF4, CZF2 or CZF3 abolish the binding of SIP1FS to alpha4IWT.	bind
448	4	1684	5	10	NULL	0	NULL			mutant	abolish			CZF2		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5073_s_199	10487759	( C) Mutations within NZF3, NZF4, CZF2 or CZF3 abolish the binding of SIP1FS to alpha4IWT.	bind
450	5	1684	5	10	NULL	0	NULL			mutant	abolish			CZF3		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5073_s_199	10487759	( C) Mutations within NZF3, NZF4, CZF2 or CZF3 abolish the binding of SIP1FS to alpha4IWT.	bind
2530	1	1684	6	10	NULL	0	NULL	SIP1	GP		bind			FS		alpha4I	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5073_s_199	10487759	( C) Mutations within NZF3, NZF4, CZF2 or CZF3 abolish the binding of SIP1FS to alpha4IWT.	bind
2531	2	1684	6	10	NULL	0	NULL			mutant	abolish			NZF3		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5073_s_199	10487759	( C) Mutations within NZF3, NZF4, CZF2 or CZF3 abolish the binding of SIP1FS to alpha4IWT.	bind
2532	3	1684	6	10	NULL	0	NULL			mutant	abolish			NZF4		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5073_s_199	10487759	( C) Mutations within NZF3, NZF4, CZF2 or CZF3 abolish the binding of SIP1FS to alpha4IWT.	bind
2533	4	1684	6	10	NULL	0	NULL			mutant	abolish			CZF2		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5073_s_199	10487759	( C) Mutations within NZF3, NZF4, CZF2 or CZF3 abolish the binding of SIP1FS to alpha4IWT.	bind
2534	5	1684	6	10	NULL	0	NULL			mutant	abolish			CZF3		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5073_s_199	10487759	( C) Mutations within NZF3, NZF4, CZF2 or CZF3 abolish the binding of SIP1FS to alpha4IWT.	bind
452	1	1685	5	10	NULL	0	NULL	Siglec	GP		bind					gangliosides 	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_41527_s_256	11553646	( c) Myelin-associated glycoprotein is a Siglec (sialic acid-specific lectin) that binds to complex gangliosides, an interaction essential for maintaining normal myelin structure ( 49,  50).	bind
453	2	1685	5	10	NULL	0	NULL	Siglec	GP		is					sialic acid-specific lectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_41527_s_256	11553646	( c) Myelin-associated glycoprotein is a Siglec (sialic acid-specific lectin) that binds to complex gangliosides, an interaction essential for maintaining normal myelin structure ( 49,  50).	bind
3304	3	1685	5	10	NULL	0	NULL	statement 1	Process		maintain					myelin structure	GP	normal			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_41527_s_256	11553646	( c) Myelin-associated glycoprotein is a Siglec (sialic acid-specific lectin) that binds to complex gangliosides, an interaction essential for maintaining normal myelin structure ( 49,  50).	bind
46150	4	1685	5	10	NULL	0	NULL	Siglec	GP		is a type of					myelin-associated glycoprotein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_41527_s_256	11553646	( c) Myelin-associated glycoprotein is a Siglec (sialic acid-specific lectin) that binds to complex gangliosides, an interaction essential for maintaining normal myelin structure ( 49,  50).	bind
2535	1	1685	6	10	NULL	0	NULL	Siglec	GP		is a type of					Myelin-associated glycoprotein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_41527_s_256	11553646	( c) Myelin-associated glycoprotein is a Siglec (sialic acid-specific lectin) that binds to complex gangliosides, an interaction essential for maintaining normal myelin structure ( 49,  50).	bind
2536	2	1685	6	10	NULL	0	NULL	Siglec	GP		is					sialic acid-specific lectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_41527_s_256	11553646	( c) Myelin-associated glycoprotein is a Siglec (sialic acid-specific lectin) that binds to complex gangliosides, an interaction essential for maintaining normal myelin structure ( 49,  50).	bind
2537	3	1685	6	10	NULL	0	NULL	statement 1	Process		bind to					complex gangliosides	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_41527_s_256	11553646	( c) Myelin-associated glycoprotein is a Siglec (sialic acid-specific lectin) that binds to complex gangliosides, an interaction essential for maintaining normal myelin structure ( 49,  50).	bind
2538	4	1685	6	10	NULL	0	NULL	statement 3	Process		maintains					mylein structure	GP	normal			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_41527_s_256	11553646	( c) Myelin-associated glycoprotein is a Siglec (sialic acid-specific lectin) that binds to complex gangliosides, an interaction essential for maintaining normal myelin structure ( 49,  50).	bind
511	1	1687	5	10	NULL	0	NULL	Smad1	GP		bind		direct			DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_541_s_107	14739937	( C) N1ICD potentiates transcriptional activity of Smad1 independent of direct binding  of Smad1 to DNA. HepG2 cells were transfected with combinations of N1ICD, Gal4, Gal4-Smad1  and Gal4-M1-Luc.	bind
512	2	1687	5	10	NULL	0	NULL	N1ICD	GP		potentiate					Smad1	GP	transcriptional activity of			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_541_s_107	14739937	( C) N1ICD potentiates transcriptional activity of Smad1 independent of direct binding  of Smad1 to DNA. HepG2 cells were transfected with combinations of N1ICD, Gal4, Gal4-Smad1  and Gal4-M1-Luc.	bind
513	3	1687	5	10	NULL	0	NULL	statement 2	Process		independent of					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_541_s_107	14739937	( C) N1ICD potentiates transcriptional activity of Smad1 independent of direct binding  of Smad1 to DNA. HepG2 cells were transfected with combinations of N1ICD, Gal4, Gal4-Smad1  and Gal4-M1-Luc.	bind
2543	1	1687	6	10	NULL	0	NULL	Smad1	GP		bind		directly			DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_541_s_107	14739937	( C) N1ICD potentiates transcriptional activity of Smad1 independent of direct binding  of Smad1 to DNA. HepG2 cells were transfected with combinations of N1ICD, Gal4, Gal4-Smad1  and Gal4-M1-Luc.	bind
2544	2	1687	6	10	NULL	0	NULL	N1ICD	GP		potentiates					Smad1	GP	transcriptional activity of			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_541_s_107	14739937	( C) N1ICD potentiates transcriptional activity of Smad1 independent of direct binding  of Smad1 to DNA. HepG2 cells were transfected with combinations of N1ICD, Gal4, Gal4-Smad1  and Gal4-M1-Luc.	bind
2545	3	1687	6	10	NULL	0	NULL	statement 2	Process		is independent of					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_541_s_107	14739937	( C) N1ICD potentiates transcriptional activity of Smad1 independent of direct binding  of Smad1 to DNA. HepG2 cells were transfected with combinations of N1ICD, Gal4, Gal4-Smad1  and Gal4-M1-Luc.	bind
514	1	1688	5	10	NULL	0	NULL	Nef	GP		bind					cholesterol	Chemical				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_100_14_8460_s_206	12824470	( c) Nef binds cholesterol  in vitro.	bind
2546	1	1688	6	10	NULL	0	NULL	Nef	GP		bind					cholesterol	Chemical				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_100_14_8460_s_206	12824470	( c) Nef binds cholesterol  in vitro.	bind
515	1	1689	5	10	NULL	0	NULL	2G12 IgG1	GP		bind					SOS gp 140	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5628_2065_s_82	12829775	( C) Negative -stain electron microscopy of unbound b12 IgG1 (top row), unbound 2G12 IgG1 (middle row), and 2G12 IgG1 bound to SOS gp 140 [bottom row (  34)] shows that the 2G12 IgG1 (bound and unbound) adopts an unusual linear shape as opposed to a classic Y shape such as that of b12.	bind
3305	2	1689	5	10	NULL	0	NULL	2G12 IgG1	GP	unbound	adopt					linear shape		unusual			NULL		NULL	NULL	NULL	NULL	gw60_science_300_5628_2065_s_82	12829775	( C) Negative -stain electron microscopy of unbound b12 IgG1 (top row), unbound 2G12 IgG1 (middle row), and 2G12 IgG1 bound to SOS gp 140 [bottom row (  34)] shows that the 2G12 IgG1 (bound and unbound) adopts an unusual linear shape as opposed to a classic Y shape such as that of b12.	bind
3306	3	1689	5	10	NULL	0	NULL	2G12 IgG1	GP	bound	adopt					linear shape		unusual			NULL		NULL	NULL	NULL	NULL	gw60_science_300_5628_2065_s_82	12829775	( C) Negative -stain electron microscopy of unbound b12 IgG1 (top row), unbound 2G12 IgG1 (middle row), and 2G12 IgG1 bound to SOS gp 140 [bottom row (  34)] shows that the 2G12 IgG1 (bound and unbound) adopts an unusual linear shape as opposed to a classic Y shape such as that of b12.	bind
3307	4	1689	5	10	NULL	0	NULL	b12	GP		adopt					Y shape		classic			NULL		NULL	NULL	NULL	NULL	gw60_science_300_5628_2065_s_82	12829775	( C) Negative -stain electron microscopy of unbound b12 IgG1 (top row), unbound 2G12 IgG1 (middle row), and 2G12 IgG1 bound to SOS gp 140 [bottom row (  34)] shows that the 2G12 IgG1 (bound and unbound) adopts an unusual linear shape as opposed to a classic Y shape such as that of b12.	bind
2549	1	1689	6	10	NULL	0	NULL	2G12 IgG1	GP		bind					SOS gp 140	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5628_2065_s_82	12829775	( C) Negative -stain electron microscopy of unbound b12 IgG1 (top row), unbound 2G12 IgG1 (middle row), and 2G12 IgG1 bound to SOS gp 140 [bottom row (  34)] shows that the 2G12 IgG1 (bound and unbound) adopts an unusual linear shape as opposed to a classic Y shape such as that of b12.	bind
2550	2	1689	6	10	NULL	0	NULL	2G12 IgG1	GP	unbound	adopts					linear shape		unusual			NULL		NULL	NULL	NULL	NULL	gw60_science_300_5628_2065_s_82	12829775	( C) Negative -stain electron microscopy of unbound b12 IgG1 (top row), unbound 2G12 IgG1 (middle row), and 2G12 IgG1 bound to SOS gp 140 [bottom row (  34)] shows that the 2G12 IgG1 (bound and unbound) adopts an unusual linear shape as opposed to a classic Y shape such as that of b12.	bind
2551	3	1689	6	10	NULL	0	NULL	2G12 IgG1	GP	bound	adopts					linear shape		unusual			NULL		NULL	NULL	NULL	NULL	gw60_science_300_5628_2065_s_82	12829775	( C) Negative -stain electron microscopy of unbound b12 IgG1 (top row), unbound 2G12 IgG1 (middle row), and 2G12 IgG1 bound to SOS gp 140 [bottom row (  34)] shows that the 2G12 IgG1 (bound and unbound) adopts an unusual linear shape as opposed to a classic Y shape such as that of b12.	bind
2552	4	1689	6	10	NULL	0	NULL	b12	GP		adopts					Y shape		classic			NULL		NULL	NULL	NULL	NULL	gw60_science_300_5628_2065_s_82	12829775	( C) Negative -stain electron microscopy of unbound b12 IgG1 (top row), unbound 2G12 IgG1 (middle row), and 2G12 IgG1 bound to SOS gp 140 [bottom row (  34)] shows that the 2G12 IgG1 (bound and unbound) adopts an unusual linear shape as opposed to a classic Y shape such as that of b12.	bind
516	1	1690	5	10	NULL	0	NULL	p300	GP		bind					Nur77	GP	minimal		MEF2-responsive element in promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_19_16_4323_s_94	10944115	( C) NFATp enhances p300 binding to the minimal MEF2-responsive element on the Nur77 promoter.	bind
517	2	1690	5	10	NULL	0	NULL	NFATp	GP		enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_16_4323_s_94	10944115	( C) NFATp enhances p300 binding to the minimal MEF2-responsive element on the Nur77 promoter.	bind
2553	1	1690	6	10	NULL	0	NULL	p300	GP		bind					Nur77	GP	minimal		MEF2-responsive element of the promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_19_16_4323_s_94	10944115	( C) NFATp enhances p300 binding to the minimal MEF2-responsive element on the Nur77 promoter.	bind
2554	2	1690	6	10	NULL	0	NULL	NFATp	GP		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_16_4323_s_94	10944115	( C) NFATp enhances p300 binding to the minimal MEF2-responsive element on the Nur77 promoter.	bind
518	1	1691	5	10	NULL	0	NULL				does not bind			AP-2 subunits		GST - synaptobrevin/VAMP	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_22_6011_s_43	11080148	( C) None of the AP-2 subunits can bind to GST - synaptobrevin/VAMP.	bind
2555	1	1691	6	10	NULL	0	NULL				does not bind			AP-2 subunits		GST - synaptobrevin/VAMP	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_22_6011_s_43	11080148	( C) None of the AP-2 subunits can bind to GST - synaptobrevin/VAMP.	bind
519	1	1692	5	10	NULL	0	NULL	SMX	Chemical		bind		direct			MHC-peptide complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_8_1591_s_201	9788973	( C) Nonreactive drugs such as SMX or  lidocaine bind directly to the MHC-peptide complex (noncovalent, processing-independent pathway).	bind
520	2	1692	5	10	NULL	0	NULL	lidocaine	Chemical		bind		direct			MHC-peptide complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_8_1591_s_201	9788973	( C) Nonreactive drugs such as SMX or  lidocaine bind directly to the MHC-peptide complex (noncovalent, processing-independent pathway).	bind
46151	3	1692	5	10	NULL	0	NULL	SMX	Chemical		is a type of					nonreactive drug	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_8_1591_s_201	9788973	( C) Nonreactive drugs such as SMX or  lidocaine bind directly to the MHC-peptide complex (noncovalent, processing-independent pathway).	bind
46152	4	1692	5	10	NULL	0	NULL	lidocaine	Chemical		is a type of					nonreactive drug	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_8_1591_s_201	9788973	( C) Nonreactive drugs such as SMX or  lidocaine bind directly to the MHC-peptide complex (noncovalent, processing-independent pathway).	bind
2556	1	1692	6	10	NULL	0	NULL	SMX	Chemical		bind		directly			MHC-peptide complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_8_1591_s_201	9788973	( C) Nonreactive drugs such as SMX or  lidocaine bind directly to the MHC-peptide complex (noncovalent, processing-independent pathway).	bind
2557	2	1692	6	10	NULL	0	NULL	lidocaine	Chemical		bind		directly			MHC-peptide complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_8_1591_s_201	9788973	( C) Nonreactive drugs such as SMX or  lidocaine bind directly to the MHC-peptide complex (noncovalent, processing-independent pathway).	bind
46169	3	1692	6	10	NULL	0	NULL	SMX	Chemical		is a type of					nonreactive drug	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_8_1591_s_201	9788973	( C) Nonreactive drugs such as SMX or  lidocaine bind directly to the MHC-peptide complex (noncovalent, processing-independent pathway).	bind
46170	4	1692	6	10	NULL	0	NULL	lidocaine	Chemical		is a type of					nonreactive drug	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_8_1591_s_201	9788973	( C) Nonreactive drugs such as SMX or  lidocaine bind directly to the MHC-peptide complex (noncovalent, processing-independent pathway).	bind
521	1	1693	5	10	NULL	0	NULL	Akt	GP	nuclear	bind		selectively			Ebp1	GP				NULL	PC12 cells	NULL	NULL	NULL	NULL	gw70_embo_25_10_2083_s_257	16642037	( C) Nuclear but not plasma membrane Akt selectively binds to Ebp1 wild type and S360D  mutant in PC12 cells.	bind
522	2	1693	5	10	NULL	0	NULL	Akt	GP	plasma membrane	does not bind		selectively			Ebp1	GP	wild type			NULL	PC12 cells	NULL	NULL	NULL	NULL	gw70_embo_25_10_2083_s_257	16642037	( C) Nuclear but not plasma membrane Akt selectively binds to Ebp1 wild type and S360D  mutant in PC12 cells.	bind
523	3	1693	5	10	NULL	0	NULL	Akt	GP	nuclear	bind		selectively			Ebp1	GP	mutant		S360D	NULL	PC12 cells	NULL	NULL	NULL	NULL	gw70_embo_25_10_2083_s_257	16642037	( C) Nuclear but not plasma membrane Akt selectively binds to Ebp1 wild type and S360D  mutant in PC12 cells.	bind
524	4	1693	5	10	NULL	0	NULL	Akt	GP	plasma membrane	does not bind		selectively			Ebp1	GP	mutant		S360D	NULL	PC12 cells	NULL	NULL	NULL	NULL	gw70_embo_25_10_2083_s_257	16642037	( C) Nuclear but not plasma membrane Akt selectively binds to Ebp1 wild type and S360D  mutant in PC12 cells.	bind
2558	1	1693	6	10	NULL	0	NULL	Akt	GP	nuclear	bind		selectively			Ebp1	GP	wild type			NULL	PC12 cells	NULL	NULL	NULL	NULL	gw70_embo_25_10_2083_s_257	16642037	( C) Nuclear but not plasma membrane Akt selectively binds to Ebp1 wild type and S360D  mutant in PC12 cells.	bind
2559	2	1693	6	10	NULL	0	NULL	Akt	GP	nuclear	bind		selectively			Ebp1	GP		S360D mutant		NULL	PC12 cells	NULL	NULL	NULL	NULL	gw70_embo_25_10_2083_s_257	16642037	( C) Nuclear but not plasma membrane Akt selectively binds to Ebp1 wild type and S360D  mutant in PC12 cells.	bind
2560	3	1693	6	10	NULL	0	NULL	Akt	GP	plasma membrane	does not bind					Ebp1	GP	wild type			NULL	PC12 cells	NULL	NULL	NULL	NULL	gw70_embo_25_10_2083_s_257	16642037	( C) Nuclear but not plasma membrane Akt selectively binds to Ebp1 wild type and S360D  mutant in PC12 cells.	bind
3229	4	1693	6	10	NULL	0	NULL	Akt	GP	plasma membrane	does not bind					Ebp1	GP		mutant S360D		NULL	PC12 cells	NULL	NULL	NULL	NULL	gw70_embo_25_10_2083_s_257	16642037	( C) Nuclear but not plasma membrane Akt selectively binds to Ebp1 wild type and S360D  mutant in PC12 cells.	bind
525	1	1695	5	10	NULL	0	NULL	Oct-2	GP		bind		specifically			CD36 octamer	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_8_1767_s_136	11937630	( C) Oct-2 specifically binds to the CD36 octamer.	bind
2562	1	1695	6	10	NULL	0	NULL	Oct-2	GP		bind		specifically			CD36 octamer	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_8_1767_s_136	11937630	( C) Oct-2 specifically binds to the CD36 octamer.	bind
526	1	1696	5	10	NULL	0	NULL	Olig2	GP		bind					 oligonucleotide	NucleicAcid			M100A	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_2_282_s_179	15655114	( C) Olig2 binds to the M100A oligonucleotide, whereas the Olig2 DNA-binding mutant Olig2-AQ  lacks this activity.	bind
527	2	1696	5	10	NULL	0	NULL	Olig2-AQ	GP	 mutant	does not bind					 oligonucleotide	NucleicAcid			M100A	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_2_282_s_179	15655114	( C) Olig2 binds to the M100A oligonucleotide, whereas the Olig2 DNA-binding mutant Olig2-AQ  lacks this activity.	bind
46269	3	1696	5	10	NULL	0	NULL	Olig2-AQ	GP		is a type of					Olig2 DNA-binding mutant 	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_2_282_s_179	15655114	( C) Olig2 binds to the M100A oligonucleotide, whereas the Olig2 DNA-binding mutant Olig2-AQ  lacks this activity.	bind
2563	1	1696	6	10	NULL	0	NULL	Olig2	GP		bind					 oligonucleotide	NucleicAcid			M100A	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_2_282_s_179	15655114	( C) Olig2 binds to the M100A oligonucleotide, whereas the Olig2 DNA-binding mutant Olig2-AQ  lacks this activity.	bind
2564	2	1696	6	10	NULL	0	NULL	Olig2-AQ	GP	mutant	does not bind					 oligonucleotide	NucleicAcid			M100A	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_2_282_s_179	15655114	( C) Olig2 binds to the M100A oligonucleotide, whereas the Olig2 DNA-binding mutant Olig2-AQ  lacks this activity.	bind
46268	3	1696	6	10	NULL	0	NULL	Olig2-AQ	GP		is a type of					Olig2 DNA binding mutant	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_2_282_s_179	15655114	( C) Olig2 binds to the M100A oligonucleotide, whereas the Olig2 DNA-binding mutant Olig2-AQ  lacks this activity.	bind
528	1	1697	5	10	NULL	0	NULL	ZONAB	GP		bind			CSD		RalA	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_1_54_s_52	15592429	( C) Only the ZONAB CSD binds RalA in a GTP-dependent manner.	bind
562	2	1697	5	10	NULL	0	NULL	statement 1	Process		dependent on					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_1_54_s_52	15592429	( C) Only the ZONAB CSD binds RalA in a GTP-dependent manner.	bind
2565	1	1697	6	10	NULL	0	NULL	ZONAB	GP		bind			CSD		RalA	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_1_54_s_52	15592429	( C) Only the ZONAB CSD binds RalA in a GTP-dependent manner.	bind
2566	2	1697	6	10	NULL	0	NULL	statement 1	Process		dependent on					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_1_54_s_52	15592429	( C) Only the ZONAB CSD binds RalA in a GTP-dependent manner.	bind
529	1	1698	5	10	NULL	0	NULL	Ins(1,4,5)P3	Chemical		bind					3G ARNO	GP		PH domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_19_3711_s_135	15359279	( C) Overlay of Ins(1,4,5)P3 bound to the 3G ARNO PH domain with the electron density corresponding to inorganic  sulfate ions from the unliganded 3G Grp1 PH domain following superposition of Calpha atoms.	bind
2567	1	1698	6	10	NULL	0	NULL	Ins(1,4,5)P3	Chemical		bind					3G ARNO	GP		PH domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_19_3711_s_135	15359279	( C) Overlay of Ins(1,4,5)P3 bound to the 3G ARNO PH domain with the electron density corresponding to inorganic  sulfate ions from the unliganded 3G Grp1 PH domain following superposition of Calpha atoms.	bind
530	1	1699	5	10	NULL	0	NULL	G-switch RNA	NucleicAcid	15N-labeled	bind					guanine	Chemical	unlabeled			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1372_s_34	15665103	( C) Overlay of the imino regions of 1H, 15N-HSQC spectra of the uniformly 15N-labeled G-switch RNA in its free form (black) and bound to unlabeled guanine (red)  at 283 K. ( D) Imino region of an 1H, 15N-HSQC spectrum of 15N-labeled guanine bound to only cytidine-13C, 15N-labeled G-switch RNA.	bind
531	2	1699	5	10	NULL	0	NULL	guanine	Chemical	15N-labeled	bind					cytidine-13C	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1372_s_34	15665103	( C) Overlay of the imino regions of 1H, 15N-HSQC spectra of the uniformly 15N-labeled G-switch RNA in its free form (black) and bound to unlabeled guanine (red)  at 283 K. ( D) Imino region of an 1H, 15N-HSQC spectrum of 15N-labeled guanine bound to only cytidine-13C, 15N-labeled G-switch RNA.	bind
46271	3	1699	5	10	NULL	0	NULL	guanine	Chemical	15N-labeled	bind					G-switch RNA	NucleicAcid	15N-labeled			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1372_s_34	15665103	( C) Overlay of the imino regions of 1H, 15N-HSQC spectra of the uniformly 15N-labeled G-switch RNA in its free form (black) and bound to unlabeled guanine (red)  at 283 K. ( D) Imino region of an 1H, 15N-HSQC spectrum of 15N-labeled guanine bound to only cytidine-13C, 15N-labeled G-switch RNA.	bind
3003	1	1699	6	10	NULL	0	NULL	G-switch RNA	NucleicAcid	15N-labeled	bind					guanine	Chemical	unlabeled			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1372_s_34	15665103	( C) Overlay of the imino regions of 1H, 15N-HSQC spectra of the uniformly 15N-labeled G-switch RNA in its free form (black) and bound to unlabeled guanine (red)  at 283 K. ( D) Imino region of an 1H, 15N-HSQC spectrum of 15N-labeled guanine bound to only cytidine-13C, 15N-labeled G-switch RNA.	bind
3004	2	1699	6	10	NULL	0	NULL	guanine 	Chemical	15N-labeled	bind					cytidine-13C	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1372_s_34	15665103	( C) Overlay of the imino regions of 1H, 15N-HSQC spectra of the uniformly 15N-labeled G-switch RNA in its free form (black) and bound to unlabeled guanine (red)  at 283 K. ( D) Imino region of an 1H, 15N-HSQC spectrum of 15N-labeled guanine bound to only cytidine-13C, 15N-labeled G-switch RNA.	bind
46270	3	1699	6	10	NULL	0	NULL	guanine	Chemical	15N-labeled	bind					G-switch RNA	NucleicAcid	15N-labeled			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_5_1372_s_34	15665103	( C) Overlay of the imino regions of 1H, 15N-HSQC spectra of the uniformly 15N-labeled G-switch RNA in its free form (black) and bound to unlabeled guanine (red)  at 283 K. ( D) Imino region of an 1H, 15N-HSQC spectrum of 15N-labeled guanine bound to only cytidine-13C, 15N-labeled G-switch RNA.	bind
532	1	1700	5	10	NULL	0	NULL	p185	GP		bind					SKP1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_17_9855_s_151	12904573	( C) p185 binds to SKP1  in an FBW6-dependent manner.	bind
533	2	1700	5	10	NULL	0	NULL	statement 1	Process		dependent on					FBW6	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_17_9855_s_151	12904573	( C) p185 binds to SKP1  in an FBW6-dependent manner.	bind
2632	1	1700	6	10	NULL	0	NULL	p185	GP		bind					SKP1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_17_9855_s_151	12904573	( C) p185 binds to SKP1  in an FBW6-dependent manner.	bind
2633	2	1700	6	10	NULL	0	NULL	statement 1	Process		is dependent on					FBW6	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_17_9855_s_151	12904573	( C) p185 binds to SKP1  in an FBW6-dependent manner.	bind
563	1	1701	5	10	NULL	0	NULL	p53	GP		bind					DNA	NucleicAcid				NULL	chimeric embryo brain extracts	NULL	NULL	NULL	NULL	gw60_embo_20_13_3402_s_156	11432828	( C) p53 gel shift analysis on chimeric embryo brain extracts demonstrates that p53 DNA binding activity correlates with the degree of  Rb - / -  chimerism.	bind
564	2	1701	5	10	NULL	0	NULL	statement 1	Process		correlates with					Rb - / - chimerism	Process	degree of			NULL	chimeric embryo brain extracts	NULL	NULL	NULL	NULL	gw60_embo_20_13_3402_s_156	11432828	( C) p53 gel shift analysis on chimeric embryo brain extracts demonstrates that p53 DNA binding activity correlates with the degree of  Rb - / -  chimerism.	bind
2634	1	1701	6	10	NULL	0	NULL	p53	GP		bind					DNA	NucleicAcid			site	NULL	chimeric embryo brain extracts	NULL	NULL	NULL	NULL	gw60_embo_20_13_3402_s_156	11432828	( C) p53 gel shift analysis on chimeric embryo brain extracts demonstrates that p53 DNA binding activity correlates with the degree of  Rb - / -  chimerism.	bind
2635	2	1701	6	10	NULL	0	NULL	statement 1	Process		correlates with 					Rb - / - chimerism	Process	degree of			NULL	chimeric embryo brain extracts	NULL	NULL	NULL	NULL	gw60_embo_20_13_3402_s_156	11432828	( C) p53 gel shift analysis on chimeric embryo brain extracts demonstrates that p53 DNA binding activity correlates with the degree of  Rb - / -  chimerism.	bind
565	1	1702	5	10	NULL	0	NULL	T3 	GP		bind					TRbeta	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5197_s_40	16549781	( C) Percentage increase in KCNH2 current in the presence of 3 muM 1-850, an antagonist  of T3 binding to TRbeta, or after overnight transfection with mutant TRbeta receptors.	bind
2636	1	1702	6	10	NULL	0	NULL	T3	GP		bind					TRbeta	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5197_s_40	16549781	( C) Percentage increase in KCNH2 current in the presence of 3 muM 1-850, an antagonist  of T3 binding to TRbeta, or after overnight transfection with mutant TRbeta receptors.	bind
566	1	1703	5	10	NULL	0	NULL	SUMO	GP		conjugate					SATB2	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_genesdev_17_24_3048_s_155	14701874	( C) PIAS1 stimulates SUMO conjugation to SATB2 in vivo.	bind
567	2	1703	5	10	NULL	0	NULL	PIAS1	GP		stimulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_24_3048_s_155	14701874	( C) PIAS1 stimulates SUMO conjugation to SATB2 in vivo.	bind
2637	1	1703	6	10	NULL	0	NULL	SUMO	GP		conjugates					SATB2	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_genesdev_17_24_3048_s_155	14701874	( C) PIAS1 stimulates SUMO conjugation to SATB2 in vivo.	bind
2638	2	1703	6	10	NULL	0	NULL	PIAS1	GP		stimulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_24_3048_s_155	14701874	( C) PIAS1 stimulates SUMO conjugation to SATB2 in vivo.	bind
568	1	1704	5	10	NULL	0	NULL	PIF3	GP		bind					G-wt probe	GP	labeled 			NULL		NULL	NULL	NULL	NULL	gw60_science_288_5467_859_s_98	10797009	( C) PIF3 binding to labeled G-wt probe is competed only by the LRE that contains a G-box ( 47).	bind
569	2	1704	5	10	NULL	0	NULL				bind				LRE G-box	G-wt probe	GP	labeled 			NULL		NULL	NULL	NULL	NULL	gw60_science_288_5467_859_s_98	10797009	( C) PIF3 binding to labeled G-wt probe is competed only by the LRE that contains a G-box ( 47).	bind
3308	3	1704	5	10	NULL	0	NULL	statement 1	Process		compete with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_288_5467_859_s_98	10797009	( C) PIF3 binding to labeled G-wt probe is competed only by the LRE that contains a G-box ( 47).	bind
2639	1	1704	6	10	NULL	0	NULL	PIF3	GP		bind					G-wt probe	GP	labeled			NULL		NULL	NULL	NULL	NULL	gw60_science_288_5467_859_s_98	10797009	( C) PIF3 binding to labeled G-wt probe is competed only by the LRE that contains a G-box ( 47).	bind
2640	2	1704	6	10	NULL	0	NULL				bind				LRE G-box	G-wt probe	GP	labeled			NULL		NULL	NULL	NULL	NULL	gw60_science_288_5467_859_s_98	10797009	( C) PIF3 binding to labeled G-wt probe is competed only by the LRE that contains a G-box ( 47).	bind
3236	3	1704	6	10	NULL	0	NULL	statement 1	Process		competes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_288_5467_859_s_98	10797009	( C) PIF3 binding to labeled G-wt probe is competed only by the LRE that contains a G-box ( 47).	bind
570	1	1705	5	10	NULL	0	NULL	PIP2	GP		bind					BAF complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_5_2824_s_90	11880634	( C) PIP2 binding by the BAF complex requires Brg, actin, and BAF53.	bind
571	2	1705	5	10	NULL	0	NULL	statement 1	Process		require					Brg	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_5_2824_s_90	11880634	( C) PIP2 binding by the BAF complex requires Brg, actin, and BAF53.	bind
572	3	1705	5	10	NULL	0	NULL	statement 1	Process		require					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_5_2824_s_90	11880634	( C) PIP2 binding by the BAF complex requires Brg, actin, and BAF53.	bind
573	4	1705	5	10	NULL	0	NULL	statement 1	Process		require					BAF53	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_5_2824_s_90	11880634	( C) PIP2 binding by the BAF complex requires Brg, actin, and BAF53.	bind
2641	1	1705	6	10	NULL	0	NULL	PIP2	GP		bind					BAF complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_5_2824_s_90	11880634	( C) PIP2 binding by the BAF complex requires Brg, actin, and BAF53.	bind
2642	2	1705	6	10	NULL	0	NULL	statement 1	Process		requires					Brg	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_5_2824_s_90	11880634	( C) PIP2 binding by the BAF complex requires Brg, actin, and BAF53.	bind
2643	3	1705	6	10	NULL	0	NULL	statement 1	Process		requires					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_5_2824_s_90	11880634	( C) PIP2 binding by the BAF complex requires Brg, actin, and BAF53.	bind
2644	4	1705	6	10	NULL	0	NULL	statement 1	Process		requires					BAF53	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_5_2824_s_90	11880634	( C) PIP2 binding by the BAF complex requires Brg, actin, and BAF53.	bind
574	1	1707	5	10	NULL	0	NULL	hTAFII130	GP		bind					HP1gamma	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_9_5919_s_125	11959914	( C) Point mutations in the HP1 box compromised hTAFII130 binding to HP1gamma.	bind
575	2	1707	5	10	NULL	0	NULL			point mutations	compromise			HP1 box		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_9_5919_s_125	11959914	( C) Point mutations in the HP1 box compromised hTAFII130 binding to HP1gamma.	bind
2645	1	1707	6	10	NULL	0	NULL	hTAFII130	GP		bind					HP1gamma	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_9_5919_s_125	11959914	( C) Point mutations in the HP1 box compromised hTAFII130 binding to HP1gamma.	bind
2646	2	1707	6	10	NULL	0	NULL			mutant	compromise			HP1 box		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_9_5919_s_125	11959914	( C) Point mutations in the HP1 box compromised hTAFII130 binding to HP1gamma.	bind
576	1	1708	5	10	NULL	0	NULL	PPAR	GP		bind									PPREs	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_embo_23_10_2083_s_115	15103326	( C) PPAR and RXR binding to PPREs  in vivo.	bind
577	2	1708	5	10	NULL	0	NULL	RXR	GP		bind									PPREs	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_embo_23_10_2083_s_115	15103326	( C) PPAR and RXR binding to PPREs  in vivo.	bind
2647	1	1708	6	10	NULL	0	NULL	PPAR	GP		bind									PPRE	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_embo_23_10_2083_s_115	15103326	( C) PPAR and RXR binding to PPREs  in vivo.	bind
2648	2	1708	6	10	NULL	0	NULL	RXR	GP		bind									PPRE	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_embo_23_10_2083_s_115	15103326	( C) PPAR and RXR binding to PPREs  in vivo.	bind
578	1	1709	5	10	NULL	0	NULL	pol	GP		bind		preferentially			PCNA	GP	monoubiquitinated			NULL	living cells	NULL	NULL	NULL	NULL	gw70_embo_23_19_3886_s_219	15359278	( C) Preferential binding of pol  to monoubiquitinated PCNA in living cells.	bind
2649	1	1709	6	10	NULL	0	NULL	Pol	GP		bind		preferentially			PCNA	GP	monoubiquitinated			NULL	living cells	NULL	NULL	NULL	NULL	gw70_embo_23_19_3886_s_219	15359278	( C) Preferential binding of pol  to monoubiquitinated PCNA in living cells.	bind
579	1	1710	5	10	NULL	0	NULL	protamine	Chemical		bind		preferentially							SAR	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_32_20_6111_s_136	15562002	( C) Preferential binding of protamine to the SAR.	bind
2650	1	1710	6	10	NULL	0	NULL	protamine	Chemical		bind		preferentially							SAR	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_32_20_6111_s_136	15562002	( C) Preferential binding of protamine to the SAR.	bind
580	1	1711	5	10	NULL	0	NULL	C4bp	GP	primate	bind					MS11	GP	Por1B strain			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_47_17142_s_174	16275906	( C) Primate C4bp binding to Por1B strains MS11 and FA1090.	bind
581	2	1711	5	10	NULL	0	NULL	C4bp	GP	primate	bind					FA1090	GP	Por1B strain			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_47_17142_s_174	16275906	( C) Primate C4bp binding to Por1B strains MS11 and FA1090.	bind
2651	2	1711	6	10	NULL	0	NULL	C4bp	GP	primate	bind					MS11	GP	Por1B strain			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_47_17142_s_174	16275906	( C) Primate C4bp binding to Por1B strains MS11 and FA1090.	bind
2652	1	1711	6	10	NULL	0	NULL	C4bp	GP	primate	bind					FA1090	GP	Por1B strain			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_47_17142_s_174	16275906	( C) Primate C4bp binding to Por1B strains MS11 and FA1090.	bind
582	1	1712	5	10	NULL	0	NULL	T-Taxol	Chemical		bind					beta-TB	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_9_5312_s_69	11309480	( c) Proposed T-Taxol conformation bound to beta-TB.	bind
2653	1	1712	6	10	NULL	0	NULL	T-Taxol	Chemical		bind					beta-TB	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_9_5312_s_69	11309480	( c) Proposed T-Taxol conformation bound to beta-TB.	bind
583	1	1713	5	10	NULL	0	NULL	ADP-ribose	Chemical		bind							yeast	macro domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_11_1911_s_173	15902274	( C) Pulldown assays for the binding of ADP-ribose to yeast and human  macro domains.	bind
584	2	1713	5	10	NULL	0	NULL	ADP-ribose	Chemical		bind							human	macro domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_11_1911_s_173	15902274	( C) Pulldown assays for the binding of ADP-ribose to yeast and human  macro domains.	bind
2654	1	1713	6	10	NULL	0	NULL	ADP-ribose	Chemical		bind							yeast	macro domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_11_1911_s_173	15902274	( C) Pulldown assays for the binding of ADP-ribose to yeast and human  macro domains.	bind
2655	2	1713	6	10	NULL	0	NULL	ADP-ribose	Chemical		bind							human	macro domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_11_1911_s_173	15902274	( C) Pulldown assays for the binding of ADP-ribose to yeast and human  macro domains.	bind
585	1	1714	5	10	NULL	0	NULL	NF-kappaB protein	GP	purified;; recombinant	bind					NF-kappaB oligo	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_15_8638_s_160	11438703	( C) Purified recombinant NF-kappaB protein binds to a consensus NF-kappaB oligo, but not to the  5.2 kb or to a consensus Stat 1 (hSIE) element.	bind
586	2	1714	5	10	NULL	0	NULL	NF-kappaB protein	GP	purified;; recombinant	does not bind									hSIE	NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_15_8638_s_160	11438703	( C) Purified recombinant NF-kappaB protein binds to a consensus NF-kappaB oligo, but not to the  5.2 kb or to a consensus Stat 1 (hSIE) element.	bind
587	3	1714	5	10	NULL	0	NULL	hSIE	GP		is					Stat 1 element	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_15_8638_s_160	11438703	( C) Purified recombinant NF-kappaB protein binds to a consensus NF-kappaB oligo, but not to the  5.2 kb or to a consensus Stat 1 (hSIE) element.	bind
2656	1	1714	6	10	NULL	0	NULL	NF-kappaB	GP	purified;;recombinant	bind					NF-kappaB oligo	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_15_8638_s_160	11438703	( C) Purified recombinant NF-kappaB protein binds to a consensus NF-kappaB oligo, but not to the  5.2 kb or to a consensus Stat 1 (hSIE) element.	bind
2657	2	1714	6	10	NULL	0	NULL	NF-kappaB	GP	purified;;recombinant	does not bind									consensus hSIE element	NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_15_8638_s_160	11438703	( C) Purified recombinant NF-kappaB protein binds to a consensus NF-kappaB oligo, but not to the  5.2 kb or to a consensus Stat 1 (hSIE) element.	bind
46097	3	1714	6	10	NULL	0	NULL	hSIE	GP		is					Stat 1 element	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_15_8638_s_160	11438703	( C) Purified recombinant NF-kappaB protein binds to a consensus NF-kappaB oligo, but not to the  5.2 kb or to a consensus Stat 1 (hSIE) element.	bind
588	1	1715	5	10	NULL	0	NULL	SRP54	GP	purified;; radiolabeled	bind					RNC-pPL86	GP	wheat germ			NULL		NULL	NULL	NULL	NULL	gw60_science_297_5585_1345_s_46	12193787	( C) Purified, radiolabeled SRP54 bound to wheat germ RNC-pPL86 or RNC-pPL86-mut was cross-linked with DSS and the reactions were analyzed by SDS-PAGE and phosphorimaging.	bind
589	2	1715	5	10	NULL	0	NULL	SRP54	GP	purified;; radiolabeled	bind					RNC-pPL86	GP	mut			NULL		NULL	NULL	NULL	NULL	gw60_science_297_5585_1345_s_46	12193787	( C) Purified, radiolabeled SRP54 bound to wheat germ RNC-pPL86 or RNC-pPL86-mut was cross-linked with DSS and the reactions were analyzed by SDS-PAGE and phosphorimaging.	bind
46099	3	1715	5	10	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_297_5585_1345_s_46	12193787	( C) Purified, radiolabeled SRP54 bound to wheat germ RNC-pPL86 or RNC-pPL86-mut was cross-linked with DSS and the reactions were analyzed by SDS-PAGE and phosphorimaging.	bind
2658	1	1715	6	10	NULL	0	NULL	SRP54	GP	purified;; radiolabeled	bind					RNC-pPL86	GP	wheat germ			NULL		NULL	NULL	NULL	NULL	gw60_science_297_5585_1345_s_46	12193787	( C) Purified, radiolabeled SRP54 bound to wheat germ RNC-pPL86 or RNC-pPL86-mut was cross-linked with DSS and the reactions were analyzed by SDS-PAGE and phosphorimaging.	bind
2659	2	1715	6	10	NULL	0	NULL	SRP54	GP	purified;; radiolabeled	bind					RNC-pPL86	GP	mutant 			NULL		NULL	NULL	NULL	NULL	gw60_science_297_5585_1345_s_46	12193787	( C) Purified, radiolabeled SRP54 bound to wheat germ RNC-pPL86 or RNC-pPL86-mut was cross-linked with DSS and the reactions were analyzed by SDS-PAGE and phosphorimaging.	bind
46101	3	1715	6	10	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_297_5585_1345_s_46	12193787	( C) Purified, radiolabeled SRP54 bound to wheat germ RNC-pPL86 or RNC-pPL86-mut was cross-linked with DSS and the reactions were analyzed by SDS-PAGE and phosphorimaging.	bind
590	1	1717	5	10	NULL	0	NULL	FGF2	GP		bind					FGFR1c-AP 	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_14_4833_s_175	15051888	( C) Quantification of FGF2 bound to FGFR1c-AP in the presence of QSulf1- or QSulf1(C-A)-treated  heparin.	bind
3117	2	1717	5	10	NULL	0	NULL	heparin	Chemical		treated with					QSulf1	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_14_4833_s_175	15051888	( C) Quantification of FGF2 bound to FGFR1c-AP in the presence of QSulf1- or QSulf1(C-A)-treated  heparin.	bind
3118	3	1717	5	10	NULL	0	NULL	heparin	Chemical		treated with					QSulf1(C-A)	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_14_4833_s_175	15051888	( C) Quantification of FGF2 bound to FGFR1c-AP in the presence of QSulf1- or QSulf1(C-A)-treated  heparin.	bind
46102	6	1717	5	10	NULL	0	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_14_4833_s_175	15051888	( C) Quantification of FGF2 bound to FGFR1c-AP in the presence of QSulf1- or QSulf1(C-A)-treated  heparin.	bind
52891	4	1717	5	10	NULL	0	NULL	statement 1	Process		in presence of					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_14_4833_s_175	15051888	( C) Quantification of FGF2 bound to FGFR1c-AP in the presence of QSulf1- or QSulf1(C-A)-treated  heparin.	bind
52892	5	1717	5	10	NULL	0	NULL	statement 1	Process		in presence of					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_14_4833_s_175	15051888	( C) Quantification of FGF2 bound to FGFR1c-AP in the presence of QSulf1- or QSulf1(C-A)-treated  heparin.	bind
2662	1	1717	6	10	NULL	0	NULL	FGF2	GP		bind					FGFR1c-AP	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_14_4833_s_175	15051888	( C) Quantification of FGF2 bound to FGFR1c-AP in the presence of QSulf1- or QSulf1(C-A)-treated  heparin.	bind
2663	2	1717	6	10	NULL	0	NULL	heparin	Chemical		treated with					QSulf1	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_14_4833_s_175	15051888	( C) Quantification of FGF2 bound to FGFR1c-AP in the presence of QSulf1- or QSulf1(C-A)-treated  heparin.	bind
3238	3	1717	6	10	NULL	0	NULL	heparin	Chemical		treated with					QSulf1(C-A)	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_14_4833_s_175	15051888	( C) Quantification of FGF2 bound to FGFR1c-AP in the presence of QSulf1- or QSulf1(C-A)-treated  heparin.	bind
46103	6	1717	6	10	NULL	0	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_14_4833_s_175	15051888	( C) Quantification of FGF2 bound to FGFR1c-AP in the presence of QSulf1- or QSulf1(C-A)-treated  heparin.	bind
52893	4	1717	6	10	NULL	0	NULL	statement 1	Process		in presence of					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_14_4833_s_175	15051888	( C) Quantification of FGF2 bound to FGFR1c-AP in the presence of QSulf1- or QSulf1(C-A)-treated  heparin.	bind
52894	5	1717	6	10	NULL	0	NULL	statement 1	Process		in presence of					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_14_4833_s_175	15051888	( C) Quantification of FGF2 bound to FGFR1c-AP in the presence of QSulf1- or QSulf1(C-A)-treated  heparin.	bind
592	1	1719	5	10	NULL	0	NULL	tau	GP		bind					AD P-tau	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_23_8864_s_50	16735465	( C) Quantitations of the tau bound to AD P-tau ( ) and to PHF ( ).	bind
593	2	1719	5	10	NULL	0	NULL	tau	GP		bind					PHF	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_23_8864_s_50	16735465	( C) Quantitations of the tau bound to AD P-tau ( ) and to PHF ( ).	bind
2665	1	1719	6	10	NULL	0	NULL	tau	GP		bind					ADP-tau	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_23_8864_s_50	16735465	( C) Quantitations of the tau bound to AD P-tau ( ) and to PHF ( ).	bind
2666	2	1719	6	10	NULL	0	NULL	tau	GP		bind					PHF	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_23_8864_s_50	16735465	( C) Quantitations of the tau bound to AD P-tau ( ) and to PHF ( ).	bind
594	1	1720	5	10	NULL	0	NULL	Rapamycin	Chemical		inhibit					Tor proteins	GP				NULL	cells replete with amino acids	NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_59_0_407_s_214	16153175	( c) Rapamycin activates Gcn2p by inhibiting the Tor proteins and, at least in part,  by dephosphorylation of Ser-577, increasing the affinity for uncharged tRNA and permitting  tRNA binding and kinase activation by basal levels of uncharged tRNAs in cells replete  with amino acids.	bind
623	2	1720	5	10	NULL	0	NULL	Rapamycin	Chemical		activate					Gcn2p	GP				NULL	cells replete with amino acids	NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_59_0_407_s_214	16153175	( c) Rapamycin activates Gcn2p by inhibiting the Tor proteins and, at least in part,  by dephosphorylation of Ser-577, increasing the affinity for uncharged tRNA and permitting  tRNA binding and kinase activation by basal levels of uncharged tRNAs in cells replete  with amino acids.	bind
624	6	1720	5	10	NULL	NULL	NULL	statement 2	Process		increase					tRNA	NucleicAcid	affinity of;;uncharged			NULL	cells replete with amino acids	NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_59_0_407_s_214	16153175	( c) Rapamycin activates Gcn2p by inhibiting the Tor proteins and, at least in part,  by dephosphorylation of Ser-577, increasing the affinity for uncharged tRNA and permitting  tRNA binding and kinase activation by basal levels of uncharged tRNAs in cells replete  with amino acids.	bind
625	7	1720	5	10	NULL	NULL	NULL	statement 2	Process		permit					tRNA	NucleicAcid	binding of			NULL	cells replete with amino acids	NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_59_0_407_s_214	16153175	( c) Rapamycin activates Gcn2p by inhibiting the Tor proteins and, at least in part,  by dephosphorylation of Ser-577, increasing the affinity for uncharged tRNA and permitting  tRNA binding and kinase activation by basal levels of uncharged tRNAs in cells replete  with amino acids.	bind
626	8	1720	5	10	NULL	0	NULL	statement 2	Process		permit					kinase	GP	activation of			NULL	cells replete with amino acids	NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_59_0_407_s_214	16153175	( c) Rapamycin activates Gcn2p by inhibiting the Tor proteins and, at least in part,  by dephosphorylation of Ser-577, increasing the affinity for uncharged tRNA and permitting  tRNA binding and kinase activation by basal levels of uncharged tRNAs in cells replete  with amino acids.	bind
3234	3	1720	5	10	NULL	0	NULL	Rapamycin	Chemical		dephosphorylate								Ser-577		NULL	cells replete with amino acids	NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_59_0_407_s_214	16153175	( c) Rapamycin activates Gcn2p by inhibiting the Tor proteins and, at least in part,  by dephosphorylation of Ser-577, increasing the affinity for uncharged tRNA and permitting  tRNA binding and kinase activation by basal levels of uncharged tRNAs in cells replete  with amino acids.	bind
52895	4	1720	5	10	NULL	0	NULL	statement 2	Process		depends on		partly			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_59_0_407_s_214	16153175	( c) Rapamycin activates Gcn2p by inhibiting the Tor proteins and, at least in part,  by dephosphorylation of Ser-577, increasing the affinity for uncharged tRNA and permitting  tRNA binding and kinase activation by basal levels of uncharged tRNAs in cells replete  with amino acids.	bind
52896	5	1720	5	10	NULL	0	NULL	statement 2	Process		depends on					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_59_0_407_s_214	16153175	( c) Rapamycin activates Gcn2p by inhibiting the Tor proteins and, at least in part,  by dephosphorylation of Ser-577, increasing the affinity for uncharged tRNA and permitting  tRNA binding and kinase activation by basal levels of uncharged tRNAs in cells replete  with amino acids.	bind
2667	1	1720	6	10	NULL	0	NULL	Rapamycin	Chemical		activates					Gcn2p	GP				NULL	cells replete with amino acids	NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_59_0_407_s_214	16153175	( c) Rapamycin activates Gcn2p by inhibiting the Tor proteins and, at least in part,  by dephosphorylation of Ser-577, increasing the affinity for uncharged tRNA and permitting  tRNA binding and kinase activation by basal levels of uncharged tRNAs in cells replete  with amino acids.	bind
2668	2	1720	6	10	NULL	0	NULL	Rapamycin	Chemical		inhibits					Tor proteins	GP				NULL	cells replete with amino acids	NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_59_0_407_s_214	16153175	( c) Rapamycin activates Gcn2p by inhibiting the Tor proteins and, at least in part,  by dephosphorylation of Ser-577, increasing the affinity for uncharged tRNA and permitting  tRNA binding and kinase activation by basal levels of uncharged tRNAs in cells replete  with amino acids.	bind
2669	3	1720	6	10	NULL	0	NULL	statement 1	Process		is dependent on					statement 2	Process				NULL	cells replete with amino acids	NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_59_0_407_s_214	16153175	( c) Rapamycin activates Gcn2p by inhibiting the Tor proteins and, at least in part,  by dephosphorylation of Ser-577, increasing the affinity for uncharged tRNA and permitting  tRNA binding and kinase activation by basal levels of uncharged tRNAs in cells replete  with amino acids.	bind
2670	4	1720	6	10	NULL	0	NULL	Rapamycin	Chemical		dephosphorylates								Ser-577		NULL	cells replete with amino acids	NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_59_0_407_s_214	16153175	( c) Rapamycin activates Gcn2p by inhibiting the Tor proteins and, at least in part,  by dephosphorylation of Ser-577, increasing the affinity for uncharged tRNA and permitting  tRNA binding and kinase activation by basal levels of uncharged tRNAs in cells replete  with amino acids.	bind
2671	5	1720	6	10	NULL	0	NULL	statement 1	Process		dependent on		partly			Statement 4	Process				NULL	cells replete with amino acids	NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_59_0_407_s_214	16153175	( c) Rapamycin activates Gcn2p by inhibiting the Tor proteins and, at least in part,  by dephosphorylation of Ser-577, increasing the affinity for uncharged tRNA and permitting  tRNA binding and kinase activation by basal levels of uncharged tRNAs in cells replete  with amino acids.	bind
2672	6	1720	6	10	NULL	NULL	NULL	statement 1	Process		increases					tRNA	NucleicAcid	affinity of;;uncharged			NULL	cells replete with amino acids	NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_59_0_407_s_214	16153175	( c) Rapamycin activates Gcn2p by inhibiting the Tor proteins and, at least in part,  by dephosphorylation of Ser-577, increasing the affinity for uncharged tRNA and permitting  tRNA binding and kinase activation by basal levels of uncharged tRNAs in cells replete  with amino acids.	bind
2673	7	1720	6	10	NULL	NULL	NULL	statement 1	Process		permits					tRNA	NucleicAcid	binding of			NULL	cells replete with amino acids	NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_59_0_407_s_214	16153175	( c) Rapamycin activates Gcn2p by inhibiting the Tor proteins and, at least in part,  by dephosphorylation of Ser-577, increasing the affinity for uncharged tRNA and permitting  tRNA binding and kinase activation by basal levels of uncharged tRNAs in cells replete  with amino acids.	bind
2674	8	1720	6	10	NULL	0	NULL	statement 1	Process		permits					kinase	GP	activation			NULL	cells replete with amino acids	NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_59_0_407_s_214	16153175	( c) Rapamycin activates Gcn2p by inhibiting the Tor proteins and, at least in part,  by dephosphorylation of Ser-577, increasing the affinity for uncharged tRNA and permitting  tRNA binding and kinase activation by basal levels of uncharged tRNAs in cells replete  with amino acids.	bind
627	1	1721	5	10	NULL	0	NULL	GATA-1	GP		bind					beta major	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_18_11760_s_201	12193659	( C) Real-time PCR ChIP analysis of binding of GATA-1, p45/NF-E2, and pol II to the beta major promoter.	bind
628	2	1721	5	10	NULL	0	NULL	p45/NF-E2	GP		bind					beta major	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_18_11760_s_201	12193659	( C) Real-time PCR ChIP analysis of binding of GATA-1, p45/NF-E2, and pol II to the beta major promoter.	bind
629	3	1721	5	10	NULL	0	NULL	pol II	GP		bind					beta major	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_18_11760_s_201	12193659	( C) Real-time PCR ChIP analysis of binding of GATA-1, p45/NF-E2, and pol II to the beta major promoter.	bind
2677	1	1721	6	10	NULL	0	NULL	GATA-1	GP		bind					beta major	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_18_11760_s_201	12193659	( C) Real-time PCR ChIP analysis of binding of GATA-1, p45/NF-E2, and pol II to the beta major promoter.	bind
2678	2	1721	6	10	NULL	0	NULL	p45/NF-E2	GP		bind					beta major	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_18_11760_s_201	12193659	( C) Real-time PCR ChIP analysis of binding of GATA-1, p45/NF-E2, and pol II to the beta major promoter.	bind
2679	3	1721	6	10	NULL	0	NULL	pol II	GP		bind					beta major	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_18_11760_s_201	12193659	( C) Real-time PCR ChIP analysis of binding of GATA-1, p45/NF-E2, and pol II to the beta major promoter.	bind
630	1	1722	5	10	NULL	0	NULL	MDM2	GP		bind					ARF	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_18_3279_s_201	16107876	( C) Relative binding affinity of MDM2 to ARF and KAP1.	bind
631	2	1722	5	10	NULL	0	NULL	MDM2	GP		bind					KAP1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_18_3279_s_201	16107876	( C) Relative binding affinity of MDM2 to ARF and KAP1.	bind
2675	1	1722	6	10	NULL	0	NULL	MDM2	GP		bind					ARF	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_18_3279_s_201	16107876	( C) Relative binding affinity of MDM2 to ARF and KAP1.	bind
2676	2	1722	6	10	NULL	0	NULL	MDM2	GP		bind					KAP1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_18_3279_s_201	16107876	( C) Relative binding affinity of MDM2 to ARF and KAP1.	bind
632	1	1723	5	10	NULL	0	NULL	JNK	GP		bind					IB1	GP	wt			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_785_s_179	16456539	( C) Relative binding of JNK, MKK7 and MLK3 to wt or mutant IB1.	bind
633	2	1723	5	10	NULL	0	NULL	JNK	GP		bind					IB1	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_785_s_179	16456539	( C) Relative binding of JNK, MKK7 and MLK3 to wt or mutant IB1.	bind
634	3	1723	5	10	NULL	0	NULL	MKK7	GP		bind					IB1	GP	wt			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_785_s_179	16456539	( C) Relative binding of JNK, MKK7 and MLK3 to wt or mutant IB1.	bind
635	4	1723	5	10	NULL	0	NULL	MKK7	GP		bind					IB1	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_785_s_179	16456539	( C) Relative binding of JNK, MKK7 and MLK3 to wt or mutant IB1.	bind
636	5	1723	5	10	NULL	0	NULL	MLK3	GP		bind					IB1	GP	wt			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_785_s_179	16456539	( C) Relative binding of JNK, MKK7 and MLK3 to wt or mutant IB1.	bind
637	6	1723	5	10	NULL	0	NULL	MLK3	GP		bind					IB1	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_785_s_179	16456539	( C) Relative binding of JNK, MKK7 and MLK3 to wt or mutant IB1.	bind
46109	7	1723	5	10	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_785_s_179	16456539	( C) Relative binding of JNK, MKK7 and MLK3 to wt or mutant IB1.	bind
46110	8	1723	5	10	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_785_s_179	16456539	( C) Relative binding of JNK, MKK7 and MLK3 to wt or mutant IB1.	bind
46111	9	1723	5	10	NULL	0	NULL	statement 5	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_785_s_179	16456539	( C) Relative binding of JNK, MKK7 and MLK3 to wt or mutant IB1.	bind
2680	1	1723	6	10	NULL	0	NULL	JNK	GP		bind					IB1	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_785_s_179	16456539	( C) Relative binding of JNK, MKK7 and MLK3 to wt or mutant IB1.	bind
2681	2	1723	6	10	NULL	0	NULL	JNK	GP		bind					IB1	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_785_s_179	16456539	( C) Relative binding of JNK, MKK7 and MLK3 to wt or mutant IB1.	bind
2682	3	1723	6	10	NULL	0	NULL	MKK7	GP		bind					IB1	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_785_s_179	16456539	( C) Relative binding of JNK, MKK7 and MLK3 to wt or mutant IB1.	bind
2683	4	1723	6	10	NULL	0	NULL	MKK7	GP		bind					IB1	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_785_s_179	16456539	( C) Relative binding of JNK, MKK7 and MLK3 to wt or mutant IB1.	bind
2684	5	1723	6	10	NULL	0	NULL	MLK3	GP		bind					IB1	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_785_s_179	16456539	( C) Relative binding of JNK, MKK7 and MLK3 to wt or mutant IB1.	bind
2685	6	1723	6	10	NULL	0	NULL	MLK3	GP		bind					IB1	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_785_s_179	16456539	( C) Relative binding of JNK, MKK7 and MLK3 to wt or mutant IB1.	bind
46112	7	1723	6	10	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_785_s_179	16456539	( C) Relative binding of JNK, MKK7 and MLK3 to wt or mutant IB1.	bind
46113	8	1723	6	10	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_785_s_179	16456539	( C) Relative binding of JNK, MKK7 and MLK3 to wt or mutant IB1.	bind
46114	9	1723	6	10	NULL	0	NULL	statement 5	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_785_s_179	16456539	( C) Relative binding of JNK, MKK7 and MLK3 to wt or mutant IB1.	bind
638	1	1724	5	10	NULL	0	NULL	RelB	GP		bind					 Bcl-xL	GP			promoter	NULL	RelA-deficient MEFs	NULL	NULL	NULL	NULL	gw70_pnas_102_41_14635_s_169	16192349	( C) RelB is bound to the  Bcl-xL promoter after TNF-alpha stimulation in RelA-deficient MEFs.	bind
639	2	1724	5	10	NULL	0	NULL	TNF-alpha	GP		stimulate					statement 1	Process				NULL	RelA-deficient MEFs	NULL	NULL	NULL	NULL	gw70_pnas_102_41_14635_s_169	16192349	( C) RelB is bound to the  Bcl-xL promoter after TNF-alpha stimulation in RelA-deficient MEFs.	bind
3122	3	1724	5	10	NULL	0	NULL	statement 2	Process		is necessary for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_41_14635_s_169	16192349	( C) RelB is bound to the  Bcl-xL promoter after TNF-alpha stimulation in RelA-deficient MEFs.	bind
2686	1	1724	6	10	NULL	0	NULL	RelB	GP		bind					Bcl-xL	GP			promoter	NULL	RelA-deficient MEFs	NULL	NULL	NULL	NULL	gw70_pnas_102_41_14635_s_169	16192349	( C) RelB is bound to the  Bcl-xL promoter after TNF-alpha stimulation in RelA-deficient MEFs.	bind
2687	2	1724	6	10	NULL	0	NULL	TNF-alpha	GP		stimulates					statement 1	Process				NULL	RelA-deficient MEFs	NULL	NULL	NULL	NULL	gw70_pnas_102_41_14635_s_169	16192349	( C) RelB is bound to the  Bcl-xL promoter after TNF-alpha stimulation in RelA-deficient MEFs.	bind
3239	3	1724	6	10	NULL	0	NULL	statement 2	Process		is necessary for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_41_14635_s_169	16192349	( C) RelB is bound to the  Bcl-xL promoter after TNF-alpha stimulation in RelA-deficient MEFs.	bind
731	1	1725	5	10	NULL	0	NULL	Bc-12	GP		bind					MDA-MB-435 cells	Cell	human			NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_49_17210_s_96	15563590	( C) Requirement of integrin alphavbeta3 activation for Bc-12 and Bc-15 binding to human breast cancer cells: MDA-MB-435  (beta3 - ) cells lack alphavbeta3 or express alphavbeta3 either in a nonactivated (beta3WT and ParentCo) or activated functional form (beta3D723R, Bone, and Lung), and BMS cells that were isolated from breast cancer patient blood.	bind
732	2	1725	5	10	NULL	0	NULL	Bc-15	GP		bind					MDA-MB-435 cells	Cell	human			NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_49_17210_s_96	15563590	( C) Requirement of integrin alphavbeta3 activation for Bc-12 and Bc-15 binding to human breast cancer cells: MDA-MB-435  (beta3 - ) cells lack alphavbeta3 or express alphavbeta3 either in a nonactivated (beta3WT and ParentCo) or activated functional form (beta3D723R, Bone, and Lung), and BMS cells that were isolated from breast cancer patient blood.	bind
734	5	1725	5	10	NULL	0	NULL	integrin alphavbeta3	GP	activation	is required for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_49_17210_s_96	15563590	( C) Requirement of integrin alphavbeta3 activation for Bc-12 and Bc-15 binding to human breast cancer cells: MDA-MB-435  (beta3 - ) cells lack alphavbeta3 or express alphavbeta3 either in a nonactivated (beta3WT and ParentCo) or activated functional form (beta3D723R, Bone, and Lung), and BMS cells that were isolated from breast cancer patient blood.	bind
735	6	1725	5	10	NULL	0	NULL	integrin alphavbeta3	GP	activation	is required for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_49_17210_s_96	15563590	( C) Requirement of integrin alphavbeta3 activation for Bc-12 and Bc-15 binding to human breast cancer cells: MDA-MB-435  (beta3 - ) cells lack alphavbeta3 or express alphavbeta3 either in a nonactivated (beta3WT and ParentCo) or activated functional form (beta3D723R, Bone, and Lung), and BMS cells that were isolated from breast cancer patient blood.	bind
3125	3	1725	5	10	NULL	0	NULL	Bc-12	GP		bind					BMS cells	Cell				NULL	from breast cancer patient blood	NULL	NULL	NULL	NULL	gw70_pnas_101_49_17210_s_96	15563590	( C) Requirement of integrin alphavbeta3 activation for Bc-12 and Bc-15 binding to human breast cancer cells: MDA-MB-435  (beta3 - ) cells lack alphavbeta3 or express alphavbeta3 either in a nonactivated (beta3WT and ParentCo) or activated functional form (beta3D723R, Bone, and Lung), and BMS cells that were isolated from breast cancer patient blood.	bind
3126	4	1725	5	10	NULL	0	NULL	Bc-15	GP		bind					BMS cells	Cell				NULL	from breast cancer patient blood	NULL	NULL	NULL	NULL	gw70_pnas_101_49_17210_s_96	15563590	( C) Requirement of integrin alphavbeta3 activation for Bc-12 and Bc-15 binding to human breast cancer cells: MDA-MB-435  (beta3 - ) cells lack alphavbeta3 or express alphavbeta3 either in a nonactivated (beta3WT and ParentCo) or activated functional form (beta3D723R, Bone, and Lung), and BMS cells that were isolated from breast cancer patient blood.	bind
3128	7	1725	5	10	NULL	0	NULL	integrin alphavbeta3	GP	activation	is required for					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_49_17210_s_96	15563590	( C) Requirement of integrin alphavbeta3 activation for Bc-12 and Bc-15 binding to human breast cancer cells: MDA-MB-435  (beta3 - ) cells lack alphavbeta3 or express alphavbeta3 either in a nonactivated (beta3WT and ParentCo) or activated functional form (beta3D723R, Bone, and Lung), and BMS cells that were isolated from breast cancer patient blood.	bind
3129	8	1725	5	10	NULL	0	NULL	integrin alphavbeta3	GP	activation	is required for					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_49_17210_s_96	15563590	( C) Requirement of integrin alphavbeta3 activation for Bc-12 and Bc-15 binding to human breast cancer cells: MDA-MB-435  (beta3 - ) cells lack alphavbeta3 or express alphavbeta3 either in a nonactivated (beta3WT and ParentCo) or activated functional form (beta3D723R, Bone, and Lung), and BMS cells that were isolated from breast cancer patient blood.	bind
46116	9	1725	5	10	NULL	0	NULL	MDA-MB-435 cells	Cell		is a type of					breast cancer cells	Cell	human			NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_49_17210_s_96	15563590	( C) Requirement of integrin alphavbeta3 activation for Bc-12 and Bc-15 binding to human breast cancer cells: MDA-MB-435  (beta3 - ) cells lack alphavbeta3 or express alphavbeta3 either in a nonactivated (beta3WT and ParentCo) or activated functional form (beta3D723R, Bone, and Lung), and BMS cells that were isolated from breast cancer patient blood.	bind
3005	1	1725	6	10	NULL	0	NULL	Bc-12	GP		bind					MDA-MB-435 (beta3 - ) cells	Cell	human			NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_49_17210_s_96	15563590	( C) Requirement of integrin alphavbeta3 activation for Bc-12 and Bc-15 binding to human breast cancer cells: MDA-MB-435  (beta3 - ) cells lack alphavbeta3 or express alphavbeta3 either in a nonactivated (beta3WT and ParentCo) or activated functional form (beta3D723R, Bone, and Lung), and BMS cells that were isolated from breast cancer patient blood.	bind
3006	2	1725	6	10	NULL	0	NULL	MDA-MB-435 (beta3 - ) cells	Cell		is a type of					breast cancer cells	Cell	human			NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_49_17210_s_96	15563590	( C) Requirement of integrin alphavbeta3 activation for Bc-12 and Bc-15 binding to human breast cancer cells: MDA-MB-435  (beta3 - ) cells lack alphavbeta3 or express alphavbeta3 either in a nonactivated (beta3WT and ParentCo) or activated functional form (beta3D723R, Bone, and Lung), and BMS cells that were isolated from breast cancer patient blood.	bind
3007	3	1725	6	10	NULL	0	NULL	Bc-15	Cell		bind					MDA-MB-435 (beta3 - ) cells	Cell	human			NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_49_17210_s_96	15563590	( C) Requirement of integrin alphavbeta3 activation for Bc-12 and Bc-15 binding to human breast cancer cells: MDA-MB-435  (beta3 - ) cells lack alphavbeta3 or express alphavbeta3 either in a nonactivated (beta3WT and ParentCo) or activated functional form (beta3D723R, Bone, and Lung), and BMS cells that were isolated from breast cancer patient blood.	bind
3024	4	1725	6	10	NULL	0	NULL	integrin alphavbeta3	GP	activation of	is required for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_49_17210_s_96	15563590	( C) Requirement of integrin alphavbeta3 activation for Bc-12 and Bc-15 binding to human breast cancer cells: MDA-MB-435  (beta3 - ) cells lack alphavbeta3 or express alphavbeta3 either in a nonactivated (beta3WT and ParentCo) or activated functional form (beta3D723R, Bone, and Lung), and BMS cells that were isolated from breast cancer patient blood.	bind
3025	5	1725	6	10	NULL	0	NULL	integrin alphavbeta3	GP	activation of	is required for					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_49_17210_s_96	15563590	( C) Requirement of integrin alphavbeta3 activation for Bc-12 and Bc-15 binding to human breast cancer cells: MDA-MB-435  (beta3 - ) cells lack alphavbeta3 or express alphavbeta3 either in a nonactivated (beta3WT and ParentCo) or activated functional form (beta3D723R, Bone, and Lung), and BMS cells that were isolated from breast cancer patient blood.	bind
46165	6	1725	6	10	NULL	0	NULL	Bc-12	GP		bind					BMS cells	Cell				NULL	breast cancer patient blood	NULL	NULL	NULL	NULL	gw70_pnas_101_49_17210_s_96	15563590	( C) Requirement of integrin alphavbeta3 activation for Bc-12 and Bc-15 binding to human breast cancer cells: MDA-MB-435  (beta3 - ) cells lack alphavbeta3 or express alphavbeta3 either in a nonactivated (beta3WT and ParentCo) or activated functional form (beta3D723R, Bone, and Lung), and BMS cells that were isolated from breast cancer patient blood.	bind
46166	7	1725	6	10	NULL	0	NULL	Bc-15	GP		bind					BMS cells	Cell				NULL	breast cancer patient blood	NULL	NULL	NULL	NULL	gw70_pnas_101_49_17210_s_96	15563590	( C) Requirement of integrin alphavbeta3 activation for Bc-12 and Bc-15 binding to human breast cancer cells: MDA-MB-435  (beta3 - ) cells lack alphavbeta3 or express alphavbeta3 either in a nonactivated (beta3WT and ParentCo) or activated functional form (beta3D723R, Bone, and Lung), and BMS cells that were isolated from breast cancer patient blood.	bind
52897	8	1725	6	10	NULL	0	NULL	integrin alphavbeta3	GP	activation of	is required for					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_49_17210_s_96	15563590	( C) Requirement of integrin alphavbeta3 activation for Bc-12 and Bc-15 binding to human breast cancer cells: MDA-MB-435  (beta3 - ) cells lack alphavbeta3 or express alphavbeta3 either in a nonactivated (beta3WT and ParentCo) or activated functional form (beta3D723R, Bone, and Lung), and BMS cells that were isolated from breast cancer patient blood.	bind
52898	9	1725	6	10	NULL	0	NULL	integrin alphavbeta3	GP	activation of	is required for					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_49_17210_s_96	15563590	( C) Requirement of integrin alphavbeta3 activation for Bc-12 and Bc-15 binding to human breast cancer cells: MDA-MB-435  (beta3 - ) cells lack alphavbeta3 or express alphavbeta3 either in a nonactivated (beta3WT and ParentCo) or activated functional form (beta3D723R, Bone, and Lung), and BMS cells that were isolated from breast cancer patient blood.	bind
737	1	1727	5	10	NULL	0	NULL	Rtt106p	GP		bind					H3	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_pnas_102_38_13410_s_195	16157874	( C) Rtt106p binds to H3 and H4  in vivo.	bind
738	2	1727	5	10	NULL	0	NULL	Rtt106p	GP		bind					H4	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_pnas_102_38_13410_s_195	16157874	( C) Rtt106p binds to H3 and H4  in vivo.	bind
2688	1	1727	6	10	NULL	0	NULL	Rtt106p	GP		bind					H3	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_pnas_102_38_13410_s_195	16157874	( C) Rtt106p binds to H3 and H4  in vivo.	bind
2689	2	1727	6	10	NULL	0	NULL	Rtt106p	GP		bind					H4	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_pnas_102_38_13410_s_195	16157874	( C) Rtt106p binds to H3 and H4  in vivo.	bind
739	1	1728	5	10	NULL	0	NULL	ADP-ribose	Chemical		bind								macro domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_11_1911_s_132	15902274	( C) Schematic representation for the binding of ADP-ribose to the  macro domain.	bind
2690	1	1728	6	10	NULL	0	NULL	ADP-ribose	Chemical		bind								macro domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_11_1911_s_132	15902274	( C) Schematic representation for the binding of ADP-ribose to the  macro domain.	bind
744	1	1729	5	10	NULL	0	NULL	YY1	GP	allele-specific	bind							unmethylated		Xist cluster	NULL	Xi of female	NULL	NULL	NULL	NULL	gw70_genomeres_16_7_901_s_127	16760423	( C) Schematic representation of allele-specific YY1 binding to the  Xist locus based on the results of  B. YY1 binds to the  Xist cluster located in the Xi of female, which is unmethylated.	bind
2691	1	1729	6	10	NULL	0	NULL	YY1	GP	allele-specific	bind							unmethylated		Xist cluster 	NULL	Xi of female	NULL	NULL	NULL	NULL	gw70_genomeres_16_7_901_s_127	16760423	( C) Schematic representation of allele-specific YY1 binding to the  Xist locus based on the results of  B. YY1 binds to the  Xist cluster located in the Xi of female, which is unmethylated.	bind
745	1	1730	5	10	NULL	0	NULL	ataxin-3	GP	derivatives	bind					VCP	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_embo_23_3_659_s_137	14749733	( C) Schematic representation of the ataxin-3 deletion mutants and summary of the data  obtained from the  in vitro assay of the binding of ataxin-3 derivatives to VCP.	bind
2692	1	1730	6	10	NULL	0	NULL	ataxin-3	GP	derivatives	bind					VCP	GP				NULL	in vitro assay	NULL	NULL	NULL	NULL	gw70_embo_23_3_659_s_137	14749733	( C) Schematic representation of the ataxin-3 deletion mutants and summary of the data  obtained from the  in vitro assay of the binding of ataxin-3 derivatives to VCP.	bind
746	1	1732	5	10	NULL	0	NULL	hSNF5	GP		regulate 					E2F targets	GP	selection of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_6_665_s_119	15769941	( C) Selection of E2F targets and mitotic controllers, regulated by hSNF5 identified  by whole-genome expression profiling.	bind
748	2	1732	5	10	NULL	0	NULL	hSNF5	GP		regulate					mitotic controllers	GP	selection of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_6_665_s_119	15769941	( C) Selection of E2F targets and mitotic controllers, regulated by hSNF5 identified  by whole-genome expression profiling.	bind
2693	1	1732	6	10	NULL	0	NULL	hSNF5	GP		regulates					E2F targets	GP	selection of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_6_665_s_119	15769941	( C) Selection of E2F targets and mitotic controllers, regulated by hSNF5 identified  by whole-genome expression profiling.	bind
2694	2	1732	6	10	NULL	0	NULL	hSNF5	GP		regulates					mitotic controllers	GP	selection of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_6_665_s_119	15769941	( C) Selection of E2F targets and mitotic controllers, regulated by hSNF5 identified  by whole-genome expression profiling.	bind
750	1	1733	5	10	NULL	0	NULL	Sema-2a-AP	GP		bind					PlexB	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_133_11_2125_s_238	16672342	( C) Sema-2a-AP binds to PlexB in the presence of 1 mM and 10 mM (inset) EDTA.	bind
3131	2	1733	5	10	NULL	0	NULL	statement 1	Process		in the presence of					EDTA	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_development_133_11_2125_s_238	16672342	( C) Sema-2a-AP binds to PlexB in the presence of 1 mM and 10 mM (inset) EDTA.	bind
2695	1	1733	6	10	NULL	0	NULL	Sema-2a-AP 	GP		bind					PlexB	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_133_11_2125_s_238	16672342	( C) Sema-2a-AP binds to PlexB in the presence of 1 mM and 10 mM (inset) EDTA.	bind
2696	2	1733	6	10	NULL	0	NULL	statement 1	Process		in presence of 					EDTA	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_development_133_11_2125_s_238	16672342	( C) Sema-2a-AP binds to PlexB in the presence of 1 mM and 10 mM (inset) EDTA.	bind
752	1	1734	5	10	NULL	0	NULL	Sens	GP		bind			Zn-finger domains		Sc	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_133_10_1979_s_232	16624856	( C) Sens binds to Sc through its Zn-finger domains.	bind
2697	1	1734	6	10	NULL	0	NULL	Sens	GP		bind			Zn-finger domain		Sc	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_133_10_1979_s_232	16624856	( C) Sens binds to Sc through its Zn-finger domains.	bind
753	1	1737	5	10	NULL	0	NULL	Src	GP		bind			SH3 domain		TRPV1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_24_4211_s_125	16319926	( C) SH3 domain of Src binds to TRPV1.	bind
2698	1	1737	6	10	NULL	0	NULL	Src	GP		bind			SH3 domain		TRPV1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_24_4211_s_125	16319926	( C) SH3 domain of Src binds to TRPV1.	bind
756	1	1738	5	10	NULL	0	NULL	Elk-1	GP	activated	recruit					mSin3A	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_22_2_281_s_251	12514134	( C) Shortly after fully fledged activation, Elk-1 recruits the co-repressor mSin3A which  binds to its DNA-binding domain (N-terminus) and attenuates histone acetylation (Yang   et al.	bind
757	2	1738	5	10	NULL	0	NULL	mSin3A	GP		bind					Elk-1	GP		DNA-binding domain (N-terminus)		NULL		NULL	NULL	NULL	NULL	gw70_embo_22_2_281_s_251	12514134	( C) Shortly after fully fledged activation, Elk-1 recruits the co-repressor mSin3A which  binds to its DNA-binding domain (N-terminus) and attenuates histone acetylation (Yang   et al.	bind
759	3	1738	5	10	NULL	0	NULL	statement 2	Process		attenuate					histone 	GP	acetylation			NULL		NULL	NULL	NULL	NULL	gw70_embo_22_2_281_s_251	12514134	( C) Shortly after fully fledged activation, Elk-1 recruits the co-repressor mSin3A which  binds to its DNA-binding domain (N-terminus) and attenuates histone acetylation (Yang   et al.	bind
46123	4	1738	5	10	NULL	0	NULL	mSin3A	GP		is a type of					co-repressor	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_22_2_281_s_251	12514134	( C) Shortly after fully fledged activation, Elk-1 recruits the co-repressor mSin3A which  binds to its DNA-binding domain (N-terminus) and attenuates histone acetylation (Yang   et al.	bind
2699	1	1738	6	10	NULL	0	NULL	mSin3A	GP		is a type of					corepressor	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_22_2_281_s_251	12514134	( C) Shortly after fully fledged activation, Elk-1 recruits the co-repressor mSin3A which  binds to its DNA-binding domain (N-terminus) and attenuates histone acetylation (Yang   et al.	bind
2700	2	1738	6	10	NULL	0	NULL	Elk1	GP	activated	recruits					mSin3A	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_22_2_281_s_251	12514134	( C) Shortly after fully fledged activation, Elk-1 recruits the co-repressor mSin3A which  binds to its DNA-binding domain (N-terminus) and attenuates histone acetylation (Yang   et al.	bind
46167	3	1738	6	10	NULL	0	NULL	mSin3A	GP		bind					Elk-1	GP		DNA-binding domain (N-terminus)		NULL		NULL	NULL	NULL	NULL	gw70_embo_22_2_281_s_251	12514134	( C) Shortly after fully fledged activation, Elk-1 recruits the co-repressor mSin3A which  binds to its DNA-binding domain (N-terminus) and attenuates histone acetylation (Yang   et al.	bind
46168	4	1738	6	10	NULL	0	NULL	statement 3	Process		attenuates					histone	GP	acetylation of			NULL		NULL	NULL	NULL	NULL	gw70_embo_22_2_281_s_251	12514134	( C) Shortly after fully fledged activation, Elk-1 recruits the co-repressor mSin3A which  binds to its DNA-binding domain (N-terminus) and attenuates histone acetylation (Yang   et al.	bind
762	1	1739	5	10	NULL	0	NULL	SKN-1	GP		bind		specifically			GST - GSK-3 	GP	C. elegans			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_102_45_16275_s_116	16251270	( C) SKN-1 binds specifically to a  C. elegans GST - GSK-3 fusion protein  in vitro.	bind
46124	2	1739	5	10	NULL	0	NULL	GSK-3	GP		is a type of					GST-fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_45_16275_s_116	16251270	( C) SKN-1 binds specifically to a  C. elegans GST - GSK-3 fusion protein  in vitro.	bind
2702	1	1739	6	10	NULL	0	NULL	SKN-1	GP		bind		specifically			GST-GSK3	GP	C. elegans  			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_102_45_16275_s_116	16251270	( C) SKN-1 binds specifically to a  C. elegans GST - GSK-3 fusion protein  in vitro.	bind
46125	2	1739	6	10	NULL	0	NULL	GSK-3	GP		is a type of					GST-fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_45_16275_s_116	16251270	( C) SKN-1 binds specifically to a  C. elegans GST - GSK-3 fusion protein  in vitro.	bind
766	1	1740	5	10	NULL	0	NULL	Smad1	GP		bind		directly							GCAT motif	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_14_3107_s_61	12136093	( C) Smad1 binds directly to the GCAT motif (and Smad4 binds weakly).	bind
768	2	1740	5	10	NULL	0	NULL	Smad4	GP		bind		weakly							GCAT motif	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_14_3107_s_61	12136093	( C) Smad1 binds directly to the GCAT motif (and Smad4 binds weakly).	bind
2703	1	1740	6	10	NULL	0	NULL	Smad1	GP		bind		directly							GCAT motif	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_14_3107_s_61	12136093	( C) Smad1 binds directly to the GCAT motif (and Smad4 binds weakly).	bind
2704	2	1740	6	10	NULL	0	NULL	Smad4	GP		bind		weakly							GCAT motif	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_14_3107_s_61	12136093	( C) Smad1 binds directly to the GCAT motif (and Smad4 binds weakly).	bind
770	1	1741	5	10	NULL	0	NULL	Smad1	GP		bind		directly							SBE III	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_14_3107_s_50	12136093	( C) Smad1, Smad3 and Smad4 bind directly to SBE III.	bind
772	2	1741	5	10	NULL	0	NULL	Smad3	GP		bind		directly							SBE III	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_14_3107_s_50	12136093	( C) Smad1, Smad3 and Smad4 bind directly to SBE III.	bind
773	3	1741	5	10	NULL	0	NULL	Smad4	GP		bind		directly							SBE III	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_14_3107_s_50	12136093	( C) Smad1, Smad3 and Smad4 bind directly to SBE III.	bind
2705	1	1741	6	10	NULL	0	NULL	Smad1	GP		bind		directly							SBE III	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_14_3107_s_50	12136093	( C) Smad1, Smad3 and Smad4 bind directly to SBE III.	bind
2706	2	1741	6	10	NULL	0	NULL	Smad3	GP		bind		directly							SBE III	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_14_3107_s_50	12136093	( C) Smad1, Smad3 and Smad4 bind directly to SBE III.	bind
2707	3	1741	6	10	NULL	0	NULL	Smad4	GP		bind		directly							SBE III	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_14_3107_s_50	12136093	( C) Smad1, Smad3 and Smad4 bind directly to SBE III.	bind
793	1	1742	5	10	NULL	0	NULL	TGF-beta	GP		induce 					p15 Ink4B	GP	transcription from		promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_19_19_5178_s_95	11013220	( C) Smad3 is required for TGF-beta-induced transcription from the p15 Ink4B promoter.	bind
794	2	1742	5	10	NULL	0	NULL	Smad3	GP		is required for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_19_5178_s_95	11013220	( C) Smad3 is required for TGF-beta-induced transcription from the p15 Ink4B promoter.	bind
2708	1	1742	6	10	NULL	0	NULL	TGF-beta	GP		induce					p15 Ink4B	GP	transcription from		promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_19_19_5178_s_95	11013220	( C) Smad3 is required for TGF-beta-induced transcription from the p15 Ink4B promoter.	bind
3390	2	1742	6	10	NULL	0	NULL	Smad3	GP		is required for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_19_5178_s_95	11013220	( C) Smad3 is required for TGF-beta-induced transcription from the p15 Ink4B promoter.	bind
795	1	1743	5	10	NULL	0	NULL	p21	GP		bind		specifically			Wnt4 gene	GP			TATA box-proximal region	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_12_1485_s_153	15964998	( C) Specific binding of p21 to the TATA box-proximal region of the  Wnt4 gene.	bind
2709	1	1743	6	10	NULL	0	NULL	p21	GP		bind		specifically			Wnt4 gene	GP			TATA box-proximal region	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_12_1485_s_153	15964998	( C) Specific binding of p21 to the TATA box-proximal region of the  Wnt4 gene.	bind
796	1	1744	5	10	NULL	0	NULL	CD1d	GP		bind					PI	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_29_10685_s_90	15243159	( c) Specificity of CD1d binding to PI and inhibition of CD1d - PI interaction by preloading  of CD1d with free PI.	bind
3132	2	1744	5	10	NULL	0	NULL	PI	Chemical	free	inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_29_10685_s_90	15243159	( c) Specificity of CD1d binding to PI and inhibition of CD1d - PI interaction by preloading  of CD1d with free PI.	bind
2710	1	1744	6	10	NULL	0	NULL	CD1d	GP		bind					PI	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_29_10685_s_90	15243159	( c) Specificity of CD1d binding to PI and inhibition of CD1d - PI interaction by preloading  of CD1d with free PI.	bind
2711	2	1744	6	10	NULL	0	NULL	PI	Chemical	free	inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_29_10685_s_90	15243159	( c) Specificity of CD1d binding to PI and inhibition of CD1d - PI interaction by preloading  of CD1d with free PI.	bind
797	1	1745	5	10	NULL	0	NULL	ss telomeric DNA	NucleicAcid		bind					POT1a N	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_21_5180_s_72	17053789	( C) Specificity of ss telomeric DNA binding to POT1a N and ( D) POT1b N.	bind
798	2	1745	5	10	NULL	0	NULL	ss telomeric DNA	NucleicAcid		bind					POT1b N	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_21_5180_s_72	17053789	( C) Specificity of ss telomeric DNA binding to POT1a N and ( D) POT1b N.	bind
2712	1	1745	6	10	NULL	0	NULL	ss telomeric DNA	NucleicAcid		bind					POT1a N	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_21_5180_s_72	17053789	( C) Specificity of ss telomeric DNA binding to POT1a N and ( D) POT1b N.	bind
2713	2	1745	6	10	NULL	0	NULL	ss telomeric DNA	NucleicAcid		bind					POT1b N	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_21_5180_s_72	17053789	( C) Specificity of ss telomeric DNA binding to POT1a N and ( D) POT1b N.	bind
802	1	1746	5	10	NULL	0	NULL	syntenin-2	GP		bind					PIP2	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_14_2556_s_44	15961997	( C) SPR sensogram showing that the binding of syntenin-2 to PIP2 increases as the PIP2 concentration in the lipid layers increases.	bind
803	2	1746	5	10	NULL	0	NULL	PIP2	GP	increase in	increases					statement 1	Process				NULL	lipid layers	NULL	NULL	NULL	NULL	gw70_embo_24_14_2556_s_44	15961997	( C) SPR sensogram showing that the binding of syntenin-2 to PIP2 increases as the PIP2 concentration in the lipid layers increases.	bind
2714	1	1746	6	10	NULL	0	NULL	syntenin-2	GP		bind					PIP2	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_14_2556_s_44	15961997	( C) SPR sensogram showing that the binding of syntenin-2 to PIP2 increases as the PIP2 concentration in the lipid layers increases.	bind
2715	2	1746	6	10	NULL	0	NULL	PIP2	GP	increased	increases					statement 1	Process				NULL	lipid layers	NULL	NULL	NULL	NULL	gw70_embo_24_14_2556_s_44	15961997	( C) SPR sensogram showing that the binding of syntenin-2 to PIP2 increases as the PIP2 concentration in the lipid layers increases.	bind
799	1	1747	5	10	NULL	0	NULL	p53RE	GP		bind					p63gamma	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_20_5487_s_199	12374749	( C) SSRP1 directly binds to the p53RE-bound p63gamma.	bind
800	2	1747	5	10	NULL	0	NULL	SSRP1	GP		bind		directly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_20_5487_s_199	12374749	( C) SSRP1 directly binds to the p53RE-bound p63gamma.	bind
2716	1	1747	6	10	NULL	0	NULL	p53RE	GP		bind					p63gamma	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_20_5487_s_199	12374749	( C) SSRP1 directly binds to the p53RE-bound p63gamma.	bind
3391	2	1747	6	10	NULL	0	NULL	SSRP1	GP		bind		directly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_20_5487_s_199	12374749	( C) SSRP1 directly binds to the p53RE-bound p63gamma.	bind
801	1	1748	5	10	NULL	0	NULL	RIS	GP		bind					FPPS	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_20_7829_s_50	16684881	( C) Stereoview detail of RIS binding to FPPS (blue).	bind
2717	1	1748	6	10	NULL	0	NULL	RIS	GP		bind					FPPS	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_20_7829_s_50	16684881	( C) Stereoview detail of RIS binding to FPPS (blue).	bind
804	1	1749	5	10	NULL	0	NULL	glucocorticoid receptor	GP		bind							MMTV		LTR	NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10788_s_224	10485904	( C) Steroid-dependent glucocorticoid receptor binding to the MMTV LTR disrupts nucleosome activating recombination but not transcription.	bind
805	2	1749	5	10	NULL	0	NULL	statement 1	Process		disrupt					recombination	Process	nucleosome activating			NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10788_s_224	10485904	( C) Steroid-dependent glucocorticoid receptor binding to the MMTV LTR disrupts nucleosome activating recombination but not transcription.	bind
806	3	1749	5	10	NULL	0	NULL	statement 1	Process		does not disrupt					transcription	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10788_s_224	10485904	( C) Steroid-dependent glucocorticoid receptor binding to the MMTV LTR disrupts nucleosome activating recombination but not transcription.	bind
46126	4	1749	5	10	NULL	0	NULL	statement 1	Process		depends on					steroid	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10788_s_224	10485904	( C) Steroid-dependent glucocorticoid receptor binding to the MMTV LTR disrupts nucleosome activating recombination but not transcription.	bind
2718	1	1749	6	10	NULL	0	NULL	glucocorticoid receptor	GP		bind							MMTV		LTR	NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10788_s_224	10485904	( C) Steroid-dependent glucocorticoid receptor binding to the MMTV LTR disrupts nucleosome activating recombination but not transcription.	bind
2719	2	1749	6	10	NULL	0	NULL	statement 1	Process		depends on					Steroid	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10788_s_224	10485904	( C) Steroid-dependent glucocorticoid receptor binding to the MMTV LTR disrupts nucleosome activating recombination but not transcription.	bind
2720	3	1749	6	10	NULL	0	NULL	statement 1	Process		disrupt					recombination	Process	nucleosome activating			NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10788_s_224	10485904	( C) Steroid-dependent glucocorticoid receptor binding to the MMTV LTR disrupts nucleosome activating recombination but not transcription.	bind
2721	4	1749	6	10	NULL	0	NULL	statement 1	Process		does not disrupt					transcription	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10788_s_224	10485904	( C) Steroid-dependent glucocorticoid receptor binding to the MMTV LTR disrupts nucleosome activating recombination but not transcription.	bind
807	1	1750	5	10	NULL	0	NULL	Mj TyrRS	GP	WT	bind					Tyr	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_17_6483_s_52	16618920	( C) Structure of the WT  Mj TyrRS ( ) bound to Tyr.	bind
2722	1	1750	6	10	NULL	0	NULL	Mj TyrRS	GP	wild type	bind					Tyr	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_17_6483_s_52	16618920	( C) Structure of the WT  Mj TyrRS ( ) bound to Tyr.	bind
808	1	1751	5	10	NULL	0	NULL	TyrRS	GP	WT	bind					Tyr	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_17_6483_s_92	16618920	( C) Structure of the WT TyrRS bound to Tyr ( ).	bind
2724	1	1751	6	10	NULL	0	NULL	TyrRS	GP	wild type	bind					Tyr	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_17_6483_s_92	16618920	( C) Structure of the WT TyrRS bound to Tyr ( ).	bind
809	1	1752	5	10	NULL	0	NULL	helicase	GP		bind					G4 DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_18_3954_s_106	12235379	( C) Summary of binding affinity, comparing  kD for each helicase binding to G4 DNA and HJ, and showing relative affinities of binding to G4 DNA and HJ.	bind
810	2	1752	5	10	NULL	0	NULL	helicase	GP		bind					HJ	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_18_3954_s_106	12235379	( C) Summary of binding affinity, comparing  kD for each helicase binding to G4 DNA and HJ, and showing relative affinities of binding to G4 DNA and HJ.	bind
2725	1	1752	6	10	NULL	0	NULL	helicase	GP		bind					G4 DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_18_3954_s_106	12235379	( C) Summary of binding affinity, comparing  kD for each helicase binding to G4 DNA and HJ, and showing relative affinities of binding to G4 DNA and HJ.	bind
2726	2	1752	6	10	NULL	0	NULL	helicase	GP		bind					HJ	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_18_3954_s_106	12235379	( C) Summary of binding affinity, comparing  kD for each helicase binding to G4 DNA and HJ, and showing relative affinities of binding to G4 DNA and HJ.	bind
811	1	1754	5	10	NULL	0	NULL	Rae-1 	GP		bind		specifically	epsilon-CD4		NKG2d	GP		CD4		NULL		NULL	NULL	NULL	NULL	gw60_science_294_5542_605_s_81	11567106	( C) Surface plasmon resonance  indicates specific binding of Rae-1 epsilon-CD4 to  NKG2d-CD4.	bind
2727	1	1754	6	10	NULL	0	NULL	Rae-1	GP		bind		specifically	epsilon-CD4		NKG2d	GP		CD4		NULL		NULL	NULL	NULL	NULL	gw60_science_294_5542_605_s_81	11567106	( C) Surface plasmon resonance  indicates specific binding of Rae-1 epsilon-CD4 to  NKG2d-CD4.	bind
1554	1	1756	5	10	NULL	0	NULL	syn1AdeltaC	GP		bind					GST-N-CFTR	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_18_10972_s_84	9724814	( C) syn1AdeltaC binds to GST-N-CFTR with an approximately 1:1 stoichiometry.	bind
2434	1	1756	7	10	NULL	0	NULL	 syn1AdeltaC	GP		bind					GST-N-CFTR	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_18_10972_s_84	9724814	( C) syn1AdeltaC binds to GST-N-CFTR with an approximately 1:1 stoichiometry.	bind
1555	1	1757	5	10	NULL	0	NULL	proteins	GP	E. coli	bind					RNA	NucleicAcid	E. coli			NULL		NULL	NULL	NULL	NULL	gw70_embo_24_19_3360_s_84	16163391	( C) Sypro ruby stain of the same gel shown in (B) indicates that both  E. coli and  B. subtilis proteins are bound to the  E. coli RNA in this assay.	bind
1556	2	1757	5	10	NULL	0	NULL	proteins	GP	B. subtilis	bind					RNA	NucleicAcid	E. coli			NULL		NULL	NULL	NULL	NULL	gw70_embo_24_19_3360_s_84	16163391	( C) Sypro ruby stain of the same gel shown in (B) indicates that both  E. coli and  B. subtilis proteins are bound to the  E. coli RNA in this assay.	bind
2438	1	1757	7	10	NULL	0	NULL	proteins	GP	E. coli 	bind					RNA	NucleicAcid	E. coli 			NULL		NULL	NULL	NULL	NULL	gw70_embo_24_19_3360_s_84	16163391	( C) Sypro ruby stain of the same gel shown in (B) indicates that both  E. coli and  B. subtilis proteins are bound to the  E. coli RNA in this assay.	bind
2439	2	1757	7	10	NULL	0	NULL	proteins	GP	B. subtilis 	bind 					RNA	NucleicAcid	E. coli 			NULL		NULL	NULL	NULL	NULL	gw70_embo_24_19_3360_s_84	16163391	( C) Sypro ruby stain of the same gel shown in (B) indicates that both  E. coli and  B. subtilis proteins are bound to the  E. coli RNA in this assay.	bind
1557	3	1758	5	10	NULL	0	NULL	TBP	GP		bind					BNA	GP			promoter	NULL	in vivo, chromatin from wild-type (WT) or mot1-42 mutant cells	NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_151	15861138	( C) TBP binding to  BNA and  URA1 promoters  in vivo was determined by ChIP using chromatin from wild-type (WT) or  mot1-42 mutant cells.	bind
1558	2	1758	5	10	NULL	0	NULL	TBP	GP		bind					URA1	GP			promoter	NULL	in vivo, chromatin from wild-type (WT) or mot1-42 mutant cells	NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_151	15861138	( C) TBP binding to  BNA and  URA1 promoters  in vivo was determined by ChIP using chromatin from wild-type (WT) or  mot1-42 mutant cells.	bind
2440	4	1758	7	10	NULL	0	NULL	 TBP 	GP		 bind					BNA	GP			promoter	NULL	  chromatin in vivo from wild-type (WT) cells	NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_151	15861138	( C) TBP binding to  BNA and  URA1 promoters  in vivo was determined by ChIP using chromatin from wild-type (WT) or  mot1-42 mutant cells.	bind
2441	5	1758	7	10	NULL	0	NULL	TBP 	GP		bind					BNA	GP			promoter	NULL	chromatin in vivo from mot1-42 mutant cells	NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_151	15861138	( C) TBP binding to  BNA and  URA1 promoters  in vivo was determined by ChIP using chromatin from wild-type (WT) or  mot1-42 mutant cells.	bind
2442	6	1758	7	10	NULL	0	NULL	TBP	GP		bind					URA1	GP			promoter	NULL	chromatin in vivo from wild-type (WT) cells	NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_151	15861138	( C) TBP binding to  BNA and  URA1 promoters  in vivo was determined by ChIP using chromatin from wild-type (WT) or  mot1-42 mutant cells.	bind
2443	7	1758	7	10	NULL	0	NULL	TBP	GP		bind 					URA1 	GP			promoter	NULL	chromatin in vivo from mot1-42 mutant cells	NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_151	15861138	( C) TBP binding to  BNA and  URA1 promoters  in vivo was determined by ChIP using chromatin from wild-type (WT) or  mot1-42 mutant cells.	bind
1559	1	1759	5	10	NULL	0	NULL	m7G	Chemical		bind					VP39 	GP	mutant	D182A		NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_13_7149_s_70	10377383	( c) The 1.83- Ang  difference electron density (2.5sigma level) of m7G bound to VP39 mutant D182A (Table  1).	bind
2445	2	1759	7	10	NULL	0	NULL	m7G	Chemical		bind					VP39	GP	mutant 	D182A		NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_13_7149_s_70	10377383	( c) The 1.83- Ang  difference electron density (2.5sigma level) of m7G bound to VP39 mutant D182A (Table  1).	bind
2446	1	1760	7	10	NULL	0	NULL	cdk2	GP		bind					p27	GP	 wild type			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_21_5159_s_176	17053782	( C) The amount of cdk2 and cdk4 bound to p27 wild type or p27T198A was measured by Western  blot analysis after immunoprecipitation against p27.	bind
2447	2	1760	7	10	NULL	0	NULL	cdk2	GP		bind					p27	GP		T198A		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_21_5159_s_176	17053782	( C) The amount of cdk2 and cdk4 bound to p27 wild type or p27T198A was measured by Western  blot analysis after immunoprecipitation against p27.	bind
2448	3	1760	7	10	NULL	0	NULL	cdk4	GP		bind					p27	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_21_5159_s_176	17053782	( C) The amount of cdk2 and cdk4 bound to p27 wild type or p27T198A was measured by Western  blot analysis after immunoprecipitation against p27.	bind
2449	4	1760	7	10	NULL	0	NULL	cdk4	GP		bind					p27	GP		T198A		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_21_5159_s_176	17053782	( C) The amount of cdk2 and cdk4 bound to p27 wild type or p27T198A was measured by Western  blot analysis after immunoprecipitation against p27.	bind
1564	1	1761	5	10	NULL	0	NULL	DLT	GP		bind					RA1-HSF	GP	radiolabeled			NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_13_3755_s_140	16893958	( C) The binding activity of DLm, and DLd, Lm and Ld, and D alone are tested by a competition  assay using an excess of each of these protein constructs to compete the binding  of DLT to radiolabeled RA1-HSF.	bind
2450	1	1761	7	10	NULL	0	NULL	DLT	GP		bind					RA1-HSF	GP	radiolabeled			NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_13_3755_s_140	16893958	( C) The binding activity of DLm, and DLd, Lm and Ld, and D alone are tested by a competition  assay using an excess of each of these protein constructs to compete the binding  of DLT to radiolabeled RA1-HSF.	bind
1565	1	1762	5	10	NULL	0	NULL	ERK2	GP		bind			CDm		MSK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_466_s_284	11157753	( C) The binding of ERK2 CDm to MSK1 was examined as in	bind
2456	1	1762	7	10	NULL	0	NULL	ERK2 	GP		bind			CDm		MSK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_466_s_284	11157753	( C) The binding of ERK2 CDm to MSK1 was examined as in	bind
1566	1	1763	5	10	NULL	0	NULL	sCD26	GP	labeled	bind					p300	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_15_8439_s_88	10900005	( C) The binding of labeled sCD26 to p300 was inhibited by an excess amount of nonlabeled sCD26.	bind
1567	2	1763	5	10	NULL	0	NULL	sCD26	GP	nonlabeled	inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_15_8439_s_88	10900005	( C) The binding of labeled sCD26 to p300 was inhibited by an excess amount of nonlabeled sCD26.	bind
2459	1	1763	7	10	NULL	0	NULL	sCD26	GP	labeled	bind					p300	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_15_8439_s_88	10900005	( C) The binding of labeled sCD26 to p300 was inhibited by an excess amount of nonlabeled sCD26.	bind
2460	2	1763	7	10	NULL	0	NULL	sCD26	GP	nonlabeled	inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_15_8439_s_88	10900005	( C) The binding of labeled sCD26 to p300 was inhibited by an excess amount of nonlabeled sCD26.	bind
1569	1	1765	5	10	NULL	0	NULL	BRG1	GP		bind					HP1beta	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_21_5797_s_120	12411497	( C) The C-terminal chromoshadow domain of HP1alpha is sufficient to promote BRG1 binding to HP1beta and HP1gamma.	bind
1570	2	1765	5	10	NULL	0	NULL	BRG1	GP		bind					HP1gamma	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_21_5797_s_120	12411497	( C) The C-terminal chromoshadow domain of HP1alpha is sufficient to promote BRG1 binding to HP1beta and HP1gamma.	bind
1571	3	1765	5	10	NULL	0	NULL	HP1alpha	GP		promote		is sufficient to	C-terminal chromoshadow domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_21_5797_s_120	12411497	( C) The C-terminal chromoshadow domain of HP1alpha is sufficient to promote BRG1 binding to HP1beta and HP1gamma.	bind
1572	4	1765	5	10	NULL	0	NULL	HP1alpha	GP		promote		is sufficient to	C-terminal chromoshadow domain		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_21_5797_s_120	12411497	( C) The C-terminal chromoshadow domain of HP1alpha is sufficient to promote BRG1 binding to HP1beta and HP1gamma.	bind
2568	1	1765	7	10	NULL	0	NULL	BRG1	GP		bind					HP1beta	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_21_5797_s_120	12411497	( C) The C-terminal chromoshadow domain of HP1alpha is sufficient to promote BRG1 binding to HP1beta and HP1gamma.	bind
2569	2	1765	7	10	NULL	0	NULL	BRG1	GP		bind					HP1gamma	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_21_5797_s_120	12411497	( C) The C-terminal chromoshadow domain of HP1alpha is sufficient to promote BRG1 binding to HP1beta and HP1gamma.	bind
2570	3	1765	7	10	NULL	0	NULL	HP1alpha	GP		promotes			 C-terminal chromoshadow domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_21_5797_s_120	12411497	( C) The C-terminal chromoshadow domain of HP1alpha is sufficient to promote BRG1 binding to HP1beta and HP1gamma.	bind
2571	4	1765	7	10	NULL	0	NULL	HP1alpha	GP		promotes			C-terminal chromoshadow domain		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_21_5797_s_120	12411497	( C) The C-terminal chromoshadow domain of HP1alpha is sufficient to promote BRG1 binding to HP1beta and HP1gamma.	bind
1573	1	1766	5	10	NULL	0	NULL	C1	GP		bind			carboxy-terminal cytoplasmic domain		TRAF proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_3_1224_s_105	11158621	( C) The C1 carboxy-terminal cytoplasmic domain can bind to TRAF proteins.	bind
2573	2	1766	7	10	NULL	0	NULL	C1 	GP		bind 			carboxy-terminal cytoplasmic domain 		TRAF proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_3_1224_s_105	11158621	( C) The C1 carboxy-terminal cytoplasmic domain can bind to TRAF proteins.	bind
1574	1	1767	5	10	NULL	0	NULL	GTP	Chemical		bind					Ypt7p	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_19_5216_s_159	10508155	( C) The catalytically active fragments with the lowest specific activity were used to follow time kinetics of hydrolysis of GTP bound to Ypt7p.	bind
2572	1	1767	7	10	NULL	0	NULL	GTP	Chemical		bind					Ypt7p	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_19_5216_s_159	10508155	( C) The catalytically active fragments with the lowest specific activity were used to follow time kinetics of hydrolysis of GTP bound to Ypt7p.	bind
1575	1	1768	5	10	NULL	0	NULL	CARM1	GP		bind			central domain		p65	GP		RHD domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_1_85_s_102	15616592	( C) The central domain of CARM1 binds to the RHD domain of p65.	bind
2576	1	1768	7	10	NULL	0	NULL	CARM1	GP		bind			central domain 		 p65	GP		RHD domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_1_85_s_102	15616592	( C) The central domain of CARM1 binds to the RHD domain of p65.	bind
2577	1	1770	7	10	NULL	0	NULL	CREM factor	GP		bind					Oxct2b	GP			promoter ( - 40/ - 20)	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_10_3401_s_211	15951513	( C) The CREM factor binds to the Oxct2b promoter ( - 40/ - 20)  in vitro.	bind
1577	1	1772	5	10	NULL	0	NULL			distal	bind				G/C element	Sp1	GP				NULL		NULL	NULL	NULL	NULL	gw60_gene_242_1_209_s_227	10721714	( C) The distal G/C element binds Sp1 in EMSA. 32P-labelled -72; -48 probe was incubated with NIH3T3 nuclear extracts, in the presence of a 100-fold molar excess of cold competitor.	bind
2578	1	1772	7	10	NULL	0	NULL			distal	bind				G/C element	Sp1	GP				NULL		NULL	NULL	NULL	NULL	gw60_gene_242_1_209_s_227	10721714	( C) The distal G/C element binds Sp1 in EMSA. 32P-labelled -72; -48 probe was incubated with NIH3T3 nuclear extracts, in the presence of a 100-fold molar excess of cold competitor.	bind
1578	1	1774	5	10	NULL	0	NULL	HOPS complex	GP		bind		directly			Vam7p	GP		PX domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_8_1579_s_191	16601699	( C) The HOPS complex binds directly to the Vam7p PX domain.	bind
2579	1	1774	7	10	NULL	0	NULL	HOPS complex	GP		binds		directly			Vam7p	GP		PX domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_8_1579_s_191	16601699	( C) The HOPS complex binds directly to the Vam7p PX domain.	bind
1579	1	1775	5	10	NULL	0	NULL	L-valine molecule	AminoAcid		bind					IleRS	GP		aminoacylation site		NULL		NULL	NULL	NULL	NULL	gw60_science_280_5363_578_s_80	9554847	( C) The L-valine molecule bound to the aminoacylation site of IleRS.	bind
2580	1	1775	7	10	NULL	0	NULL	 L-valine	AminoAcid		bind					IleRS	GP		 aminoacylation site		NULL		NULL	NULL	NULL	NULL	gw60_science_280_5363_578_s_80	9554847	( C) The L-valine molecule bound to the aminoacylation site of IleRS.	bind
1580	1	1776	5	10	NULL	0	NULL	L13	AminoAcid	mutation of 	change					U1C	GP	conformation of 			NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_41_14841_s_183	15465910	( C) The L13 mutation causes a U1C conformational change (blue square rather than blue  oval), which binds poorly to RNA. U1 RNA therefore has a tendency to adopt the low-temperature  conformation as in  A, which allows the ps5'' to interact with the 5' end of U1 (double arrow)  and compete with pre-mRNA base-pairing.	bind
1581	2	1776	5	10	NULL	0	NULL	statement 1	Process		bind		poorly			RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_41_14841_s_183	15465910	( C) The L13 mutation causes a U1C conformational change (blue square rather than blue  oval), which binds poorly to RNA. U1 RNA therefore has a tendency to adopt the low-temperature  conformation as in  A, which allows the ps5'' to interact with the 5' end of U1 (double arrow)  and compete with pre-mRNA base-pairing.	bind
1584	3	1776	5	10	NULL	0	NULL	U1 RNA	NucleicAcid		adopt		tendency to			low-temperature conformation	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_41_14841_s_183	15465910	( C) The L13 mutation causes a U1C conformational change (blue square rather than blue  oval), which binds poorly to RNA. U1 RNA therefore has a tendency to adopt the low-temperature  conformation as in  A, which allows the ps5'' to interact with the 5' end of U1 (double arrow)  and compete with pre-mRNA base-pairing.	bind
1585	4	1776	5	10	NULL	0	NULL	ps5''	GP		interact with					U1	NucleicAcid		5' end		NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_41_14841_s_183	15465910	( C) The L13 mutation causes a U1C conformational change (blue square rather than blue  oval), which binds poorly to RNA. U1 RNA therefore has a tendency to adopt the low-temperature  conformation as in  A, which allows the ps5'' to interact with the 5' end of U1 (double arrow)  and compete with pre-mRNA base-pairing.	bind
1587	5	1776	5	10	NULL	0	NULL	statement 3	Process		allows					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_41_14841_s_183	15465910	( C) The L13 mutation causes a U1C conformational change (blue square rather than blue  oval), which binds poorly to RNA. U1 RNA therefore has a tendency to adopt the low-temperature  conformation as in  A, which allows the ps5'' to interact with the 5' end of U1 (double arrow)  and compete with pre-mRNA base-pairing.	bind
1590	6	1776	5	10	NULL	0	NULL	ps5''	GP		compete with					pre-mRNA base-pairing	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_41_14841_s_183	15465910	( C) The L13 mutation causes a U1C conformational change (blue square rather than blue  oval), which binds poorly to RNA. U1 RNA therefore has a tendency to adopt the low-temperature  conformation as in  A, which allows the ps5'' to interact with the 5' end of U1 (double arrow)  and compete with pre-mRNA base-pairing.	bind
1591	7	1776	5	10	NULL	0	NULL	statement 3	Process		allows					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_41_14841_s_183	15465910	( C) The L13 mutation causes a U1C conformational change (blue square rather than blue  oval), which binds poorly to RNA. U1 RNA therefore has a tendency to adopt the low-temperature  conformation as in  A, which allows the ps5'' to interact with the 5' end of U1 (double arrow)  and compete with pre-mRNA base-pairing.	bind
2581	2	1776	7	10	NULL	0	NULL	statement 1	Process		bind		poorly			RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_41_14841_s_183	15465910	( C) The L13 mutation causes a U1C conformational change (blue square rather than blue  oval), which binds poorly to RNA. U1 RNA therefore has a tendency to adopt the low-temperature  conformation as in  A, which allows the ps5'' to interact with the 5' end of U1 (double arrow)  and compete with pre-mRNA base-pairing.	bind
2582	3	1776	7	10	NULL	0	NULL	ps5''	GP		bind					U1	NucleicAcid			5' end	NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_41_14841_s_183	15465910	( C) The L13 mutation causes a U1C conformational change (blue square rather than blue  oval), which binds poorly to RNA. U1 RNA therefore has a tendency to adopt the low-temperature  conformation as in  A, which allows the ps5'' to interact with the 5' end of U1 (double arrow)  and compete with pre-mRNA base-pairing.	bind
2583	1	1776	7	10	NULL	0	NULL	L13 	AminoAcid	mutation of	change					U1C 	GP	conformation of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_41_14841_s_183	15465910	( C) The L13 mutation causes a U1C conformational change (blue square rather than blue  oval), which binds poorly to RNA. U1 RNA therefore has a tendency to adopt the low-temperature  conformation as in  A, which allows the ps5'' to interact with the 5' end of U1 (double arrow)  and compete with pre-mRNA base-pairing.	bind
2584	4	1776	7	10	NULL	0	NULL	U1 RNA	NucleicAcid		adopts					low-temperature conformation	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_41_14841_s_183	15465910	( C) The L13 mutation causes a U1C conformational change (blue square rather than blue  oval), which binds poorly to RNA. U1 RNA therefore has a tendency to adopt the low-temperature  conformation as in  A, which allows the ps5'' to interact with the 5' end of U1 (double arrow)  and compete with pre-mRNA base-pairing.	bind
2585	5	1776	7	10	NULL	0	NULL	statement 4	Process		allows					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_41_14841_s_183	15465910	( C) The L13 mutation causes a U1C conformational change (blue square rather than blue  oval), which binds poorly to RNA. U1 RNA therefore has a tendency to adopt the low-temperature  conformation as in  A, which allows the ps5'' to interact with the 5' end of U1 (double arrow)  and compete with pre-mRNA base-pairing.	bind
2586	6	1776	7	10	NULL	0	NULL	 ps5''	GP		compete with					pre-mRNA base-pairing	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_41_14841_s_183	15465910	( C) The L13 mutation causes a U1C conformational change (blue square rather than blue  oval), which binds poorly to RNA. U1 RNA therefore has a tendency to adopt the low-temperature  conformation as in  A, which allows the ps5'' to interact with the 5' end of U1 (double arrow)  and compete with pre-mRNA base-pairing.	bind
61570	7	1776	7	10	NULL	0	NULL	statement 4	Process		allows					statement 6	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_101_41_14841_s_183	15465910	( C) The L13 mutation causes a U1C conformational change (blue square rather than blue  oval), which binds poorly to RNA. U1 RNA therefore has a tendency to adopt the low-temperature  conformation as in  A, which allows the ps5'' to interact with the 5' end of U1 (double arrow)  and compete with pre-mRNA base-pairing.	bind
1595	1	1777	5	10	NULL	0	NULL	Nbp2	GP		bind			N-terminal domain (residues 1 115)		Ptc1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_2_302_s_164	14685261	( C) The Nbp2 N-terminal domain (residues 1 115) binds Ptc1.	bind
2587	2	1777	7	10	NULL	0	NULL	Nbp2	GP		binds			N-terminal domain (residues 1 115) 		Ptc1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_2_302_s_164	14685261	( C) The Nbp2 N-terminal domain (residues 1 115) binds Ptc1.	bind
1597	1	1778	5	10	NULL	0	NULL	NCT	GP		bind			TM		PSCT	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_24_4738_s_79	15549135	( C) The NCT TM binds PSCT also in the context of VSVG-EGFP, another type I protein.	bind
2588	1	1778	7	10	NULL	0	NULL	NCT	GP		bind			 TM		PSCT	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_24_4738_s_79	15549135	( C) The NCT TM binds PSCT also in the context of VSVG-EGFP, another type I protein.	bind
1598	1	1780	5	10	NULL	0	NULL	VAP-1	GP	oligosaccahride modifications	bind					lectin-like molecule	GP	unknown			NULL	lymphocytes	NULL	NULL	NULL	NULL	gw60_embo_20_15_3893_s_117	11483492	( C) The oligosaccahride modifications of VAP-1 (purple extensions) can bind to an unknown lectin-like molecule (yellow) on lymphocytes.	bind
2591	1	1780	7	10	NULL	0	NULL	VAP-1 	GP	oligosaccahride modifications	bind					lectin-like molecule	GP	unknown			NULL	lymphocytes	NULL	NULL	NULL	NULL	gw60_embo_20_15_3893_s_117	11483492	( C) The oligosaccahride modifications of VAP-1 (purple extensions) can bind to an unknown lectin-like molecule (yellow) on lymphocytes.	bind
2593	1	1781	7	10	NULL	0	NULL	Dlg1	GP		bind					E4-ORF1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_6_1406_s_98	16511562	( C) The PDZ1+2 conformational unit is necessary and sufficient to mediate binding of  Dlg1 to E4-ORF1.	bind
2595	2	1781	7	10	NULL	0	NULL	PDZ1+2	GP		is necessary for			conformational unit		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_6_1406_s_98	16511562	( C) The PDZ1+2 conformational unit is necessary and sufficient to mediate binding of  Dlg1 to E4-ORF1.	bind
1602	1	1782	5	10	NULL	0	NULL	PACS-1	GP	recombinant HIS-tagged	bind			furin-binding region (115 255)		polycystin-2 fragment	GP	recombinant GST-tagged	741 871 		NULL	in vitro	NULL	NULL	NULL	NULL	gw70_embo_24_4_705_s_42	15692563	( C) The recombinant HIS-tagged furin-binding region of PACS-1 (HIS.PACS-1115 255) binds a recombinant GST-tagged polycystin-2 fragment containing amino acids 741  871 (GST. PKD2741 871)  in vitro (upper panel).	bind
2601	1	1782	7	10	NULL	0	NULL	PACS-1	GP	recombinant HIS-tagged	bind			furin-binding region HIS.PACS-1115 255		polycystin-2 fragment	GP	recombinant GST-tagged 	amino acids 741 to 871		NULL	in vitro	NULL	NULL	NULL	NULL	gw70_embo_24_4_705_s_42	15692563	( C) The recombinant HIS-tagged furin-binding region of PACS-1 (HIS.PACS-1115 255) binds a recombinant GST-tagged polycystin-2 fragment containing amino acids 741  871 (GST. PKD2741 871)  in vitro (upper panel).	bind
2603	1	1783	7	10	NULL	0	NULL	mTAb1	GP		bind					mTOR	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_13_7772_s_120	9636226	( C) The relative amounts of mTAb1 bound to mTOR were determined by laser densitometry.	bind
1608	1	1784	5	10	NULL	0	NULL	PIAS3	GP	mutant	does not bind			RING domain		p300	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_1_99_s_147	14691252	( C) The RING domain mutant PIAS3 cannot bind to p300.	bind
2605	1	1784	7	10	NULL	0	NULL	PIAS3 	GP	mutant	does not bind			RING domain 		p300	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_1_99_s_147	14691252	( C) The RING domain mutant PIAS3 cannot bind to p300.	bind
1609	1	1785	5	10	NULL	0	NULL	fibronectin	GP		bind					beta1 integrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_2_692_s_77	10639141	( c) The same experiment as  a in the presence of 2 mg/ml RGD peptide, which inhibits fibronectin binding to the beta1 integrin ( 19,  20).	bind
1610	2	1785	5	10	NULL	0	NULL	RGD peptide	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_2_692_s_77	10639141	( c) The same experiment as  a in the presence of 2 mg/ml RGD peptide, which inhibits fibronectin binding to the beta1 integrin ( 19,  20).	bind
2607	1	1785	7	10	NULL	0	NULL	fibronectin	GP		bind					beta1 integrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_2_692_s_77	10639141	( c) The same experiment as  a in the presence of 2 mg/ml RGD peptide, which inhibits fibronectin binding to the beta1 integrin ( 19,  20).	bind
2609	2	1785	7	10	NULL	0	NULL	RGD peptide	GP		inhibits					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_2_692_s_77	10639141	( c) The same experiment as  a in the presence of 2 mg/ml RGD peptide, which inhibits fibronectin binding to the beta1 integrin ( 19,  20).	bind
1612	1	1786	5	10	NULL	0	NULL	FGFR	GP		bind			D2		FGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_750_s_20	12730587	( C) The second (D2) and third (D3) Ig-like extracellular domains of FGFR bind to FGF; the cofactor heparin binds to a positively charged region in D2.	bind
1613	2	1786	5	10	NULL	0	NULL	D2	GP		is					second Ig-like extracellular domains	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_750_s_20	12730587	( C) The second (D2) and third (D3) Ig-like extracellular domains of FGFR bind to FGF; the cofactor heparin binds to a positively charged region in D2.	bind
1614	3	1786	5	10	NULL	0	NULL	FGFR	GP		bind			D3		FGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_750_s_20	12730587	( C) The second (D2) and third (D3) Ig-like extracellular domains of FGFR bind to FGF; the cofactor heparin binds to a positively charged region in D2.	bind
1616	4	1786	5	10	NULL	0	NULL	D3	GP		is					third Ig-like extracellular domains	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_750_s_20	12730587	( C) The second (D2) and third (D3) Ig-like extracellular domains of FGFR bind to FGF; the cofactor heparin binds to a positively charged region in D2.	bind
1618	5	1786	5	10	NULL	0	NULL	heparin	GP	cofactor	bind					D2	GP		positively charged region		NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_750_s_20	12730587	( C) The second (D2) and third (D3) Ig-like extracellular domains of FGFR bind to FGF; the cofactor heparin binds to a positively charged region in D2.	bind
2610	1	1786	7	10	NULL	0	NULL	FGFR	GP		bind			D2 domain		FGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_750_s_20	12730587	( C) The second (D2) and third (D3) Ig-like extracellular domains of FGFR bind to FGF; the cofactor heparin binds to a positively charged region in D2.	bind
2611	2	1786	7	10	NULL	0	NULL	Heparin	GP	cofactor	bind					D2	GP		positively charged region 		NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_750_s_20	12730587	( C) The second (D2) and third (D3) Ig-like extracellular domains of FGFR bind to FGF; the cofactor heparin binds to a positively charged region in D2.	bind
50332	3	1786	7	10	NULL	0	NULL	FGFR	GP		bind			D3 domain		FGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_750_s_20	12730587	( C) The second (D2) and third (D3) Ig-like extracellular domains of FGFR bind to FGF; the cofactor heparin binds to a positively charged region in D2.	bind
50333	4	1786	7	10	NULL	0	NULL	D2	GP		is					second Ig-like extracellular domains 	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_750_s_20	12730587	( C) The second (D2) and third (D3) Ig-like extracellular domains of FGFR bind to FGF; the cofactor heparin binds to a positively charged region in D2.	bind
50334	5	1786	7	10	NULL	0	NULL	D3	GP		is					third Ig-like extracellular domain	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_750_s_20	12730587	( C) The second (D2) and third (D3) Ig-like extracellular domains of FGFR bind to FGF; the cofactor heparin binds to a positively charged region in D2.	bind
1611	1	1788	5	10	NULL	0	NULL	SMN complex	GP		bind					U1 snRNA	NucleicAcid		SL1		NULL		NULL	NULL	NULL	NULL	gw60_embo_21_5_1188_s_100	11867547	( C) The SMN complex binding to the SL1 of U1 snRNA is sequence specific.	bind
2574	2	1788	5	10	NULL	0	NULL	statement 1	Process		occurs in					sequence specific manner	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_5_1188_s_100	11867547	( C) The SMN complex binding to the SL1 of U1 snRNA is sequence specific.	bind
2612	1	1788	7	10	NULL	0	NULL	SMN complex	GP		bind					U1 snRNA	NucleicAcid		SL1 		NULL		NULL	NULL	NULL	NULL	gw60_embo_21_5_1188_s_100	11867547	( C) The SMN complex binding to the SL1 of U1 snRNA is sequence specific.	bind
2613	2	1788	7	10	NULL	0	NULL	statement 1	Process		occur in 					sequence specific manner	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_5_1188_s_100	11867547	( C) The SMN complex binding to the SL1 of U1 snRNA is sequence specific.	bind
2736	1	1789	5	10	NULL	0	NULL	SMN complex	GP		bind					U1 snRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_5_1188_s_71	11867547	( C) The SMN complex binding to U1 snRNA is independent of Sm core assembly.	bind
2737	2	1789	5	10	NULL	0	NULL	statement 1	Process		independent of					Sm core assembly	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_5_1188_s_71	11867547	( C) The SMN complex binding to U1 snRNA is independent of Sm core assembly.	bind
2614	1	1789	7	10	NULL	0	NULL	SMN complex	GP		bind					 U1 snRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_5_1188_s_71	11867547	( C) The SMN complex binding to U1 snRNA is independent of Sm core assembly.	bind
2615	2	1789	7	10	NULL	0	NULL	statement 1	Process		is independent of					Sm core assembly	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_5_1188_s_71	11867547	( C) The SMN complex binding to U1 snRNA is independent of Sm core assembly.	bind
2746	1	1790	5	10	NULL	0	NULL	ssDNA	NucleicAcid		bind					hRad54	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_6_1346_s_143	11884632	( C) The ssDNA binding of hRad54 and hRad54B.	bind
2747	2	1790	5	10	NULL	0	NULL	ssDNA	NucleicAcid		bind					hRad54B	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_6_1346_s_143	11884632	( C) The ssDNA binding of hRad54 and hRad54B.	bind
2616	1	1790	7	10	NULL	0	NULL	ssDNA	NucleicAcid		bind					hRad54	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_6_1346_s_143	11884632	( C) The ssDNA binding of hRad54 and hRad54B.	bind
2617	2	1790	7	10	NULL	0	NULL	ssDNA	NucleicAcid		bind					hRad54B	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_6_1346_s_143	11884632	( C) The ssDNA binding of hRad54 and hRad54B.	bind
2749	1	1791	5	10	NULL	0	NULL	TIF32	GP		bind			CTD		18S rRNA	NucleicAcid	biotinylated			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_6_786_s_192	12651896	( C) The TIF32-CTD binds to biotinylated 18S rRNA in Northwestern assays.	bind
2618	1	1791	7	10	NULL	0	NULL	TIF32	GP		bind			CTD		18S rRNA	NucleicAcid	biotinylated			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_6_786_s_192	12651896	( C) The TIF32-CTD binds to biotinylated 18S rRNA in Northwestern assays.	bind
2619	1	1792	7	10	NULL	0	NULL	Ku 	GP		bind					TRF1	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_22_2807_s_123	11090128	( C) The TRF1 homodimer bound to internal telomeric tracts with Ku bound to TRF1.	bind
2620	2	1792	7	10	NULL	0	NULL	TRF1 homodimer	GP		binds to							internal 	telomeric tracts		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_22_2807_s_123	11090128	( C) The TRF1 homodimer bound to internal telomeric tracts with Ku bound to TRF1.	bind
2762	1	1793	5	10	NULL	0	NULL	TRX	GP		bind			SET domain		histone	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_17_2197_s_20	11544176	( C) The TRX SET domain binds to a histone-affinity matrix.	bind
2621	1	1793	7	10	NULL	0	NULL	 TRX	GP		bind			SET domain		histone	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_17_2197_s_20	11544176	( C) The TRX SET domain binds to a histone-affinity matrix.	bind
2764	1	1794	5	10	NULL	0	NULL	FANCG	GP		bind					CYP2E1	GP				NULL		NULL	NULL	NULL	NULL	gw60_carcinogenesis_23_1_67_s_114	11756225	( C) The upper panel shows the binding of FANCG to CYP2E1.	bind
2622	1	1794	7	10	NULL	0	NULL	FANCG	GP		bind					 CYP2E1	GP				NULL		NULL	NULL	NULL	NULL	gw60_carcinogenesis_23_1_67_s_114	11756225	( C) The upper panel shows the binding of FANCG to CYP2E1.	bind
2767	1	1795	5	10	NULL	0	NULL	holo-TFIID	GP		bind					TBP antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5447_2153_s_94	10591646	( C) The yellow mesh shows the density difference between the holo-TFIID and TFIID that is bound to the TBP antibody.	bind
2768	2	1795	5	10	NULL	0	NULL	TFIID	GP		bind					TBP antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5447_2153_s_94	10591646	( C) The yellow mesh shows the density difference between the holo-TFIID and TFIID that is bound to the TBP antibody.	bind
2623	1	1795	7	10	NULL	0	NULL	holo-TFIID	GP		bind					TBP antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5447_2153_s_94	10591646	( C) The yellow mesh shows the density difference between the holo-TFIID and TFIID that is bound to the TBP antibody.	bind
2624	2	1795	7	10	NULL	0	NULL	TFIID	GP		bind					TBP antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5447_2153_s_94	10591646	( C) The yellow mesh shows the density difference between the holo-TFIID and TFIID that is bound to the TBP antibody.	bind
2776	1	1796	5	10	NULL	0	NULL	PIC	GP		bind									Ad origin of DNA replication	NULL		NULL	NULL	NULL	NULL	gw60_gene_236_1_1_s_193	10433960	( C) This PIC binds the Ad origin of DNA replication (the 5' attached TP was omitted for simplification), most likely in a irregular, bent DNA structure.	bind
2778	2	1796	5	10	NULL	0	NULL	statement 1	Process		occurs					DNA structure	NucleicAcid	irregular bent			NULL		NULL	NULL	NULL	NULL	gw60_gene_236_1_1_s_193	10433960	( C) This PIC binds the Ad origin of DNA replication (the 5' attached TP was omitted for simplification), most likely in a irregular, bent DNA structure.	bind
2625	1	1796	7	10	NULL	0	NULL	PIC	GP		bind									Ad origin of DNA replication	NULL		NULL	NULL	NULL	NULL	gw60_gene_236_1_1_s_193	10433960	( C) This PIC binds the Ad origin of DNA replication (the 5' attached TP was omitted for simplification), most likely in a irregular, bent DNA structure.	bind
2626	2	1796	7	10	NULL	0	NULL	statement 1	Process		occurs					 DNA structure	NucleicAcid	 irregular bent			NULL		NULL	NULL	NULL	NULL	gw60_gene_236_1_1_s_193	10433960	( C) This PIC binds the Ad origin of DNA replication (the 5' attached TP was omitted for simplification), most likely in a irregular, bent DNA structure.	bind
2780	1	1797	5	10	NULL	0	NULL	THP-1 	GP		bind					MCP-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_289_5482_1202_s_105	10947989	( C) THP-1 cell receptor binding of MCP-3 and  MCP-3(5-76).	bind
2781	2	1797	5	10	NULL	0	NULL	THP-1	GP		bind					MCP-3	GP		5-76		NULL		NULL	NULL	NULL	NULL	gw60_science_289_5482_1202_s_105	10947989	( C) THP-1 cell receptor binding of MCP-3 and  MCP-3(5-76).	bind
50335	3	1797	5	10	NULL	0	NULL	THP-1	GP		is a type of					cell receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_289_5482_1202_s_105	10947989	( C) THP-1 cell receptor binding of MCP-3 and  MCP-3(5-76).	bind
2627	1	1797	7	10	NULL	0	NULL	THP-1	GP		bind					MCP-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_289_5482_1202_s_105	10947989	( C) THP-1 cell receptor binding of MCP-3 and  MCP-3(5-76).	bind
2628	2	1797	7	10	NULL	0	NULL	THP-1	GP		bind					MCP-3	GP		5-76		NULL		NULL	NULL	NULL	NULL	gw60_science_289_5482_1202_s_105	10947989	( C) THP-1 cell receptor binding of MCP-3 and  MCP-3(5-76).	bind
50337	3	1797	7	10	NULL	0	NULL	THP-1	GP		is a type of					cell receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_289_5482_1202_s_105	10947989	( C) THP-1 cell receptor binding of MCP-3 and  MCP-3(5-76).	bind
2783	1	1799	5	10	NULL	0	NULL	Tpr	GP		does not bind					importin alpha/beta-NLS complexes	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_1_31_s_419	9531546	( C) Tpr does not bind to importin  alpha/beta-NLS complexes.	bind
2629	1	1799	7	10	NULL	0	NULL	Tpr	GP		does not bind					importin alpha/beta-NLS complexes	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_1_31_s_419	9531546	( C) Tpr does not bind to importin  alpha/beta-NLS complexes.	bind
2787	1	1800	5	10	NULL	0	NULL	translesion polymerase	GP		bind					recA	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_37_0_31_s_295	14616055	( c) Translesion polymerase binds to recA and related proteins.	bind
2788	2	1800	5	10	NULL	0	NULL	translesion polymerase	GP		bind					related proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_37_0_31_s_295	14616055	( c) Translesion polymerase binds to recA and related proteins.	bind
2630	1	1800	7	10	NULL	0	NULL	Translesion polymerase	GP		bind					recA	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_37_0_31_s_295	14616055	( c) Translesion polymerase binds to recA and related proteins.	bind
2631	2	1800	7	10	NULL	0	NULL	Translesion polymerase	GP	 	bind					recA related proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_37_0_31_s_295	14616055	( c) Translesion polymerase binds to recA and related proteins.	bind
2789	1	1801	5	10	NULL	0	NULL	Tre1	GP		bind					Bsd2	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_embo_25_4_662_s_141	16456538	( C) Tre1 binds Bsd2  in vivo.	bind
1926	1	1801	7	10	NULL	0	NULL	 Tre1	GP		bind					Bsd2	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_embo_25_4_662_s_141	16456538	( C) Tre1 binds Bsd2  in vivo.	bind
2790	1	1802	5	10	NULL	0	NULL	tRNA	NucleicAcid		bind		directly			Exp5	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_22_6216_s_177	12426393	( C) tRNA can bind directly to Exp5.	bind
1927	1	1802	7	10	NULL	0	NULL	tRNA	NucleicAcid		bind		directly			Exp5	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_22_6216_s_177	12426393	( C) tRNA can bind directly to Exp5.	bind
2791	1	1803	5	10	NULL	0	NULL	p65	GP	unphosphorylated	bind					HDAC1	GP				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_25_10_1991_s_285	15192014	( C) Unphosphorylated p65 but not phosphorylated (S536) p65 binds to HDAC1 and 3.	bind
2792	2	1803	5	10	NULL	0	NULL	p65	GP	unphosphorylated	bind					HDAC3	GP				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_25_10_1991_s_285	15192014	( C) Unphosphorylated p65 but not phosphorylated (S536) p65 binds to HDAC1 and 3.	bind
2793	3	1803	5	10	NULL	0	NULL	p65	GP	phosphorylated	does not bind			S536		HDAC1	GP				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_25_10_1991_s_285	15192014	( C) Unphosphorylated p65 but not phosphorylated (S536) p65 binds to HDAC1 and 3.	bind
2794	4	1803	5	10	NULL	0	NULL	p65	GP	phosphorylated	does not bind			S536		HDAC3	GP				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_25_10_1991_s_285	15192014	( C) Unphosphorylated p65 but not phosphorylated (S536) p65 binds to HDAC1 and 3.	bind
1928	1	1803	7	10	NULL	0	NULL	p65	GP	unphosphorylated	bind					 HDAC1	GP				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_25_10_1991_s_285	15192014	( C) Unphosphorylated p65 but not phosphorylated (S536) p65 binds to HDAC1 and 3.	bind
1929	2	1803	7	10	NULL	0	NULL	p65	GP	unphosphorylated	binds to					HDAC3	GP				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_25_10_1991_s_285	15192014	( C) Unphosphorylated p65 but not phosphorylated (S536) p65 binds to HDAC1 and 3.	bind
1930	3	1803	7	10	NULL	0	NULL	p65	GP	phosphorylated 	does not bind			S536		HDAC1	GP				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_25_10_1991_s_285	15192014	( C) Unphosphorylated p65 but not phosphorylated (S536) p65 binds to HDAC1 and 3.	bind
1931	4	1803	7	10	NULL	0	NULL	p65	GP	phosphorylated 	does not bind			S536		HDAC3	GP				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_25_10_1991_s_285	15192014	( C) Unphosphorylated p65 but not phosphorylated (S536) p65 binds to HDAC1 and 3.	bind
2820	1	1806	5	10	NULL	0	NULL	eIF4E	GP		bind					m7G-Sepharose	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_52_18105_s_57	15601771	( c) Western blot of eIF4E remaining bound to m7G-Sepharose upon competition with various concentrations of m7GTP or RTP.	bind
2821	2	1806	5	10	NULL	0	NULL	eIF4E	GP		bind					m7GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_52_18105_s_57	15601771	( c) Western blot of eIF4E remaining bound to m7G-Sepharose upon competition with various concentrations of m7GTP or RTP.	bind
2822	3	1806	5	10	NULL	0	NULL	eIF4E	GP		bind					RTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_52_18105_s_57	15601771	( c) Western blot of eIF4E remaining bound to m7G-Sepharose upon competition with various concentrations of m7GTP or RTP.	bind
2823	4	1806	5	10	NULL	0	NULL	statement 2	Process		compete					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_52_18105_s_57	15601771	( c) Western blot of eIF4E remaining bound to m7G-Sepharose upon competition with various concentrations of m7GTP or RTP.	bind
3201	5	1806	5	10	NULL	0	NULL	statement 3	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_52_18105_s_57	15601771	( c) Western blot of eIF4E remaining bound to m7G-Sepharose upon competition with various concentrations of m7GTP or RTP.	bind
1932	1	1806	7	10	NULL	0	NULL	eIF4E	GP		bind to					m7G-Sepharose	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_52_18105_s_57	15601771	( c) Western blot of eIF4E remaining bound to m7G-Sepharose upon competition with various concentrations of m7GTP or RTP.	bind
1933	2	1806	7	10	NULL	0	NULL	eIF4E	GP		bind to					m7GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_52_18105_s_57	15601771	( c) Western blot of eIF4E remaining bound to m7G-Sepharose upon competition with various concentrations of m7GTP or RTP.	bind
1934	3	1806	7	10	NULL	0	NULL	eIF4E	GP		bind to					RTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_52_18105_s_57	15601771	( c) Western blot of eIF4E remaining bound to m7G-Sepharose upon competition with various concentrations of m7GTP or RTP.	bind
2207	4	1806	7	10	NULL	0	NULL	statement 2	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_52_18105_s_57	15601771	( c) Western blot of eIF4E remaining bound to m7G-Sepharose upon competition with various concentrations of m7GTP or RTP.	bind
2208	5	1806	7	10	NULL	0	NULL	statement 3	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_52_18105_s_57	15601771	( c) Western blot of eIF4E remaining bound to m7G-Sepharose upon competition with various concentrations of m7GTP or RTP.	bind
1935	1	1809	7	10	NULL	0	NULL	GST. PRIC285	GP		bind					GST-PPARalpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_18_11836_s_138	12189208	( C) [35]Methionine-labeled full-length PRIC285 generated by  in vitro translation was incubated with GSH-Sepharose beads bound with purified  E. coli-expressed GST-PPARalpha or GST. PRIC285 bound to PPARalpha in the absence of ligand, and the addition of ligand increased the binding  2-fold.	bind
1936	2	1809	7	10	NULL	0	NULL	statement 1	Process		occurs in absence of 					ligand	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_18_11836_s_138	12189208	( C) [35]Methionine-labeled full-length PRIC285 generated by  in vitro translation was incubated with GSH-Sepharose beads bound with purified  E. coli-expressed GST-PPARalpha or GST. PRIC285 bound to PPARalpha in the absence of ligand, and the addition of ligand increased the binding  2-fold.	bind
1937	3	1809	7	10	NULL	0	NULL	ligand	GP	presence of 	increase					statement 1	Process	 			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_18_11836_s_138	12189208	( C) [35]Methionine-labeled full-length PRIC285 generated by  in vitro translation was incubated with GSH-Sepharose beads bound with purified  E. coli-expressed GST-PPARalpha or GST. PRIC285 bound to PPARalpha in the absence of ligand, and the addition of ligand increased the binding  2-fold.	bind
2824	1	1810	5	10	NULL	0	NULL	Galphai	GP		does not bind		directly			ERalpha	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_49_17126_s_172	15569929	( C)Galphai does not bind directly to ERalpha.	bind
1938	1	1810	7	10	NULL	0	NULL	Galphai	GP		does not bind		directly			ERalpha	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_49_17126_s_172	15569929	( C)Galphai does not bind directly to ERalpha.	bind
2825	1	1812	5	10	NULL	0	NULL	Swi/nf	GP		bind					GAL1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_embo_23_20_4040_s_74	15385957	( C, D) Binding of Swi/nf to the  GAL1 and  GAL7 promoters, respectively.	bind
2826	2	1812	5	10	NULL	0	NULL	Swi/nf	GP		bind					GAL7	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_embo_23_20_4040_s_74	15385957	( C, D) Binding of Swi/nf to the  GAL1 and  GAL7 promoters, respectively.	bind
1939	1	1812	7	10	NULL	0	NULL	 Swi/nf	GP		bind					 GAL1 	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_embo_23_20_4040_s_74	15385957	( C, D) Binding of Swi/nf to the  GAL1 and  GAL7 promoters, respectively.	bind
1940	2	1812	7	10	NULL	0	NULL	Swi/nf	GP		bind					GAL7 	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_embo_23_20_4040_s_74	15385957	( C, D) Binding of Swi/nf to the  GAL1 and  GAL7 promoters, respectively.	bind
2827	1	1813	5	10	NULL	0	NULL	TNF-alpha	GP		degrade					IkappaB-alpha	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_22_2668_s_130	16260493	( C,D) IkappaB-alpha degradation and JNK phosphorylation by TNF-alpha ( C) or IL-1 ( D) were analyzed by immunoblotting with antibodies specific for IkappaB-alpha and phospho-JNK, respectively.	bind
2828	2	1813	5	10	NULL	0	NULL	IL-1	GP		degrade					IkappaB-alpha	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_22_2668_s_130	16260493	( C,D) IkappaB-alpha degradation and JNK phosphorylation by TNF-alpha ( C) or IL-1 ( D) were analyzed by immunoblotting with antibodies specific for IkappaB-alpha and phospho-JNK, respectively.	bind
2829	3	1813	5	10	NULL	0	NULL	TNF-alpha	GP		phosphorylate					JNK	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_22_2668_s_130	16260493	( C,D) IkappaB-alpha degradation and JNK phosphorylation by TNF-alpha ( C) or IL-1 ( D) were analyzed by immunoblotting with antibodies specific for IkappaB-alpha and phospho-JNK, respectively.	bind
2830	4	1813	5	10	NULL	0	NULL	IL-1	GP		phosphorylate					JNK	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_22_2668_s_130	16260493	( C,D) IkappaB-alpha degradation and JNK phosphorylation by TNF-alpha ( C) or IL-1 ( D) were analyzed by immunoblotting with antibodies specific for IkappaB-alpha and phospho-JNK, respectively.	bind
1941	1	1813	7	10	NULL	0	NULL	JNK 	GP		phosphorylated by					TNF-alpha	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_22_2668_s_130	16260493	( C,D) IkappaB-alpha degradation and JNK phosphorylation by TNF-alpha ( C) or IL-1 ( D) were analyzed by immunoblotting with antibodies specific for IkappaB-alpha and phospho-JNK, respectively.	bind
1942	2	1813	7	10	NULL	0	NULL	JNK	GP		phosphorylated by					 IL-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_22_2668_s_130	16260493	( C,D) IkappaB-alpha degradation and JNK phosphorylation by TNF-alpha ( C) or IL-1 ( D) were analyzed by immunoblotting with antibodies specific for IkappaB-alpha and phospho-JNK, respectively.	bind
50340	3	1813	7	10	NULL	0	NULL	TNF-alpha	GP		degrade					IkappaB-alpha	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_22_2668_s_130	16260493	( C,D) IkappaB-alpha degradation and JNK phosphorylation by TNF-alpha ( C) or IL-1 ( D) were analyzed by immunoblotting with antibodies specific for IkappaB-alpha and phospho-JNK, respectively.	bind
50341	4	1813	7	10	NULL	0	NULL	IL-1	GP		degrade					IkappaB-alpha	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_22_2668_s_130	16260493	( C,D) IkappaB-alpha degradation and JNK phosphorylation by TNF-alpha ( C) or IL-1 ( D) were analyzed by immunoblotting with antibodies specific for IkappaB-alpha and phospho-JNK, respectively.	bind
2831	1	1815	5	10	NULL	0	NULL	R anti-CD21 antibody	GP		bind					CD21	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_16_10641_s_190	12122212	( Center) Flow cytometry showing binding of R anti-CD21 antibody to CD21 and CD21mut (dark lines) but not to L cells transfected with vector alone.	bind
2832	2	1815	5	10	NULL	0	NULL	R anti-CD21 antibody	GP		bind					CD21mut	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_16_10641_s_190	12122212	( Center) Flow cytometry showing binding of R anti-CD21 antibody to CD21 and CD21mut (dark lines) but not to L cells transfected with vector alone.	bind
2833	3	1815	5	10	NULL	0	NULL	R anti-CD21 antibody	GP		does not bind					L cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_16_10641_s_190	12122212	( Center) Flow cytometry showing binding of R anti-CD21 antibody to CD21 and CD21mut (dark lines) but not to L cells transfected with vector alone.	bind
1943	1	1815	7	10	NULL	0	NULL	R anti-CD21 antibody	GP		bind 					CD21	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_16_10641_s_190	12122212	( Center) Flow cytometry showing binding of R anti-CD21 antibody to CD21 and CD21mut (dark lines) but not to L cells transfected with vector alone.	bind
1944	2	1815	7	10	NULL	0	NULL	R anti-CD21 antibody	GP		bind 					CD21mut	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_16_10641_s_190	12122212	( Center) Flow cytometry showing binding of R anti-CD21 antibody to CD21 and CD21mut (dark lines) but not to L cells transfected with vector alone.	bind
1945	3	1815	7	10	NULL	0	NULL	R anti-CD21 antibody	GP		does not bind					L cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_16_10641_s_190	12122212	( Center) Flow cytometry showing binding of R anti-CD21 antibody to CD21 and CD21mut (dark lines) but not to L cells transfected with vector alone.	bind
2834	1	1817	5	10	NULL	0	NULL	HeLa cells	Cell		transfected with					pCR3-uniTM-huPrP	GP		1 - 253		NULL		NULL	NULL	NULL	NULL	gw60_embo_20_21_5863_s_72	11689427	( D - F) Binding of GST::huPrP23 - 230 by HeLa cells transfected with pCR3-uniTM-huPrP1 - 253.	bind
2835	2	1817	5	10	NULL	0	NULL	statement 1	Process		bind					GST::huPrP	GP		23 - 230		NULL		NULL	NULL	NULL	NULL	gw60_embo_20_21_5863_s_72	11689427	( D - F) Binding of GST::huPrP23 - 230 by HeLa cells transfected with pCR3-uniTM-huPrP1 - 253.	bind
1946	1	1817	7	10	NULL	0	NULL	 HeLa cells	Cell		transfected with					pCR3-uniTM-huPrP	GP		1 - 253		NULL		NULL	NULL	NULL	NULL	gw60_embo_20_21_5863_s_72	11689427	( D - F) Binding of GST::huPrP23 - 230 by HeLa cells transfected with pCR3-uniTM-huPrP1 - 253.	bind
46218	2	1817	7	10	NULL	0	NULL	GST::huPrP	GP		bind			23 - 230 		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_21_5863_s_72	11689427	( D - F) Binding of GST::huPrP23 - 230 by HeLa cells transfected with pCR3-uniTM-huPrP1 - 253.	bind
2837	1	1822	5	10	NULL	0	NULL	CI-MPRs	GP	mutant	bind					GST-GGA2	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_292_5522_1716_s_47	11387476	( D to  G) Binding of mutant CI-MPRs to GST-GGA2.	bind
1954	1	1822	7	10	NULL	0	NULL	CI-MPRs	GP	mutant	bind					GST-GGA2	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_292_5522_1716_s_47	11387476	( D to  G) Binding of mutant CI-MPRs to GST-GGA2.	bind
2838	1	1824	5	10	NULL	0	NULL	palF58 protein	GP		bind			S86P		PalH	GP		C-terminal region		NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_102_34_12141_s_133	16099830	( D)  In vitro binding of  palF58 (S86P) and  palF60 (I331K) proteins to the C-terminal region of PalH.	bind
2839	2	1824	5	10	NULL	0	NULL	palF60 protein	GP		bind			I331K		PalH	GP		C-terminal region		NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_102_34_12141_s_133	16099830	( D)  In vitro binding of  palF58 (S86P) and  palF60 (I331K) proteins to the C-terminal region of PalH.	bind
1955	1	1824	7	10	NULL	0	NULL	palF58 proteins	GP		bind			S86P		PalH	GP		C-terminal region of		NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_102_34_12141_s_133	16099830	( D)  In vitro binding of  palF58 (S86P) and  palF60 (I331K) proteins to the C-terminal region of PalH.	bind
1956	2	1824	7	10	NULL	0	NULL	palF60 proteins	GP		bind			I331K		PalH	GP		C-terminal region of		NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_102_34_12141_s_133	16099830	( D)  In vitro binding of  palF58 (S86P) and  palF60 (I331K) proteins to the C-terminal region of PalH.	bind
2840	1	1825	5	10	NULL	0	NULL	Fez1 proteins	GP		bind					EF1gamma protein	GP		N-terminal		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_pnas_98_18_10374_s_144	11504921	( D)  In vitro binding of Fez1 proteins to N-terminal EF1gamma protein.	bind
1957	1	1825	7	10	NULL	0	NULL	Fez1 proteins	GP		bind					EF1gamma protein	GP		N-terminal		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_pnas_98_18_10374_s_144	11504921	( D)  In vitro binding of Fez1 proteins to N-terminal EF1gamma protein.	bind
2841	1	1826	5	10	NULL	0	NULL	U1 snRNA	NucleicAcid		bind					U1 snRNP proteins	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_8_2493_s_202	15863726	( D)  In vitro U1 snRNA binding of U1 snRNP proteins.	bind
1958	1	1826	7	10	NULL	0	NULL	U1 snRNA	NucleicAcid		binds to					U1 snRNP proteins	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_8_2493_s_202	15863726	( D)  In vitro U1 snRNA binding of U1 snRNP proteins.	bind
2842	1	1828	5	10	NULL	0	NULL	5'' vRNA	NucleicAcid		bind					polymerase	GP		PB1 sequence		NULL		NULL	NULL	NULL	NULL	gw70_embo_22_5_1188_s_73	12606583	( D) 5'' vRNA and 5' cRNA bind to the same PB1 sequence in the polymerase.	bind
2843	2	1828	5	10	NULL	0	NULL	5' cRNA	NucleicAcid		bind					polymerase	GP		PB1 sequence		NULL		NULL	NULL	NULL	NULL	gw70_embo_22_5_1188_s_73	12606583	( D) 5'' vRNA and 5' cRNA bind to the same PB1 sequence in the polymerase.	bind
1959	1	1828	7	10	NULL	0	NULL	5'' vRNA	NucleicAcid		bind					polymerase	GP		PB1 sequence		NULL		NULL	NULL	NULL	NULL	gw70_embo_22_5_1188_s_73	12606583	( D) 5'' vRNA and 5' cRNA bind to the same PB1 sequence in the polymerase.	bind
1960	2	1828	7	10	NULL	0	NULL	5' cRNA	NucleicAcid		bind					polymerase	GP		PB1 sequence		NULL		NULL	NULL	NULL	NULL	gw70_embo_22_5_1188_s_73	12606583	( D) 5'' vRNA and 5' cRNA bind to the same PB1 sequence in the polymerase.	bind
2844	1	1829	5	10	NULL	0	NULL	STAT5A	GP		bind					beta-casein	GP			promoter containing a GAS element	NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_12_8253_s_124	12048235	( D) A gel-shift assay demonstrating the DNA-binding activity of the STAT5A with the beta-casein promoter, which contained a GAS element.	bind
1961	1	1829	7	10	NULL	0	NULL	STAT5A	GP		bind					 beta-casein	GP			promoter containing a GAS element	NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_12_8253_s_124	12048235	( D) A gel-shift assay demonstrating the DNA-binding activity of the STAT5A with the beta-casein promoter, which contained a GAS element.	bind
2845	1	1830	5	10	NULL	0	NULL	PACS-1 protein	GP	recombinant	contains			amino acids 85-280		MBP	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_4_705_s_44	15692563	( D) A recombinant PACS-1 protein (amino acids 85 280) containing the maltose-binding  protein (MBP) (MBP.PACS-185 280) immobilizes polycystin-2 from mouse kidney lysates, demonstrating that native polycystin-2  recognizes and binds PACS-1.	bind
2846	2	1830	5	10	NULL	0	NULL	MBP 	GP		is					maltose-binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_4_705_s_44	15692563	( D) A recombinant PACS-1 protein (amino acids 85 280) containing the maltose-binding  protein (MBP) (MBP.PACS-185 280) immobilizes polycystin-2 from mouse kidney lysates, demonstrating that native polycystin-2  recognizes and binds PACS-1.	bind
2847	3	1830	5	10	NULL	0	NULL	statement 1	Process		immobilizes					polycystin-2	GP				NULL	mouse kidney lysates	NULL	NULL	NULL	NULL	gw70_embo_24_4_705_s_44	15692563	( D) A recombinant PACS-1 protein (amino acids 85 280) containing the maltose-binding  protein (MBP) (MBP.PACS-185 280) immobilizes polycystin-2 from mouse kidney lysates, demonstrating that native polycystin-2  recognizes and binds PACS-1.	bind
2848	4	1830	5	10	NULL	0	NULL	polycystin-2	GP	native	recognizes					PACS-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_4_705_s_44	15692563	( D) A recombinant PACS-1 protein (amino acids 85 280) containing the maltose-binding  protein (MBP) (MBP.PACS-185 280) immobilizes polycystin-2 from mouse kidney lysates, demonstrating that native polycystin-2  recognizes and binds PACS-1.	bind
2849	5	1830	5	10	NULL	0	NULL	polycystin-2	GP	native	bind					PACS-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_4_705_s_44	15692563	( D) A recombinant PACS-1 protein (amino acids 85 280) containing the maltose-binding  protein (MBP) (MBP.PACS-185 280) immobilizes polycystin-2 from mouse kidney lysates, demonstrating that native polycystin-2  recognizes and binds PACS-1.	bind
1962	1	1830	7	10	NULL	0	NULL	PACS-1 protein	GP	recombinant	contains			amino acids 85 - 280		MBP	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_4_705_s_44	15692563	( D) A recombinant PACS-1 protein (amino acids 85 280) containing the maltose-binding  protein (MBP) (MBP.PACS-185 280) immobilizes polycystin-2 from mouse kidney lysates, demonstrating that native polycystin-2  recognizes and binds PACS-1.	bind
1963	2	1830	7	10	NULL	0	NULL	MBP	GP		is					maltose-binding protein 	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_4_705_s_44	15692563	( D) A recombinant PACS-1 protein (amino acids 85 280) containing the maltose-binding  protein (MBP) (MBP.PACS-185 280) immobilizes polycystin-2 from mouse kidney lysates, demonstrating that native polycystin-2  recognizes and binds PACS-1.	bind
1964	3	1830	7	10	NULL	0	NULL	statement 1	Process		immobilizes					polycystin-2	GP				NULL	mouse kidney lysates	NULL	NULL	NULL	NULL	gw70_embo_24_4_705_s_44	15692563	( D) A recombinant PACS-1 protein (amino acids 85 280) containing the maltose-binding  protein (MBP) (MBP.PACS-185 280) immobilizes polycystin-2 from mouse kidney lysates, demonstrating that native polycystin-2  recognizes and binds PACS-1.	bind
46276	4	1830	7	10	NULL	0	NULL	polycystin-2	GP	native	recognize					PACS-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_4_705_s_44	15692563	( D) A recombinant PACS-1 protein (amino acids 85 280) containing the maltose-binding  protein (MBP) (MBP.PACS-185 280) immobilizes polycystin-2 from mouse kidney lysates, demonstrating that native polycystin-2  recognizes and binds PACS-1.	bind
46277	5	1830	7	10	NULL	0	NULL	polycystin-2	GP	native	bind					PACS-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_4_705_s_44	15692563	( D) A recombinant PACS-1 protein (amino acids 85 280) containing the maltose-binding  protein (MBP) (MBP.PACS-185 280) immobilizes polycystin-2 from mouse kidney lysates, demonstrating that native polycystin-2  recognizes and binds PACS-1.	bind
2850	1	1831	5	10	NULL	0	NULL	c-Rel homodimer	GP		bind			RHR		IL-2	GP			promoter containing CD28 response element	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_18_2138_s_128	16166378	( D) A structural model of the c-Rel RHR homodimer bound to the CD28 response element  from the IL-2 promoter is shown (Huang et al. 2001 ).	bind
2210	1	1831	7	10	NULL	0	NULL	c-Rel homodimer	GP		bind			RHR		IL-2	GP			CD28 response element in the promoter of 	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_18_2138_s_128	16166378	( D) A structural model of the c-Rel RHR homodimer bound to the CD28 response element  from the IL-2 promoter is shown (Huang et al. 2001 ).	bind
2851	1	1832	5	10	NULL	0	NULL	phosphatase	GP		activate					E2F	GP	binding of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_pnas_99_22_14200_s_77	12379745	( D) Activation of E2F binding by phosphatase treatment in vitro.	bind
2211	1	1832	7	10	NULL	0	NULL	phosphatase	GP		activates					E2F	GP	binding of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_pnas_99_22_14200_s_77	12379745	( D) Activation of E2F binding by phosphatase treatment in vitro.	bind
2852	1	1833	5	10	NULL	0	NULL	Akt	GP	active	bind					Ebp1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_10_2083_s_144	16642037	( D) Active Akt binds Ebp1.	bind
2212	1	1833	7	10	NULL	0	NULL	Akt	GP	active	bind					Ebp1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_10_2083_s_144	16642037	( D) Active Akt binds Ebp1.	bind
2853	1	1834	5	10	NULL	0	NULL	Rabkinesin-6	GP		bind			motor domain		MT	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_science_279_5350_580_s_45	9438855	( D) Adenosine triphosphate-dependent MT-binding activity of Rabkinesin-6 motor domain.	bind
2854	2	1834	5	10	NULL	0	NULL	statement 1	Process		is dependent on					Adenosine triphosphate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_279_5350_580_s_45	9438855	( D) Adenosine triphosphate-dependent MT-binding activity of Rabkinesin-6 motor domain.	bind
2213	1	1834	7	10	NULL	0	NULL	Rabkinesin-6 	GP		binds			motor domain		MT	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_science_279_5350_580_s_45	9438855	( D) Adenosine triphosphate-dependent MT-binding activity of Rabkinesin-6 motor domain.	bind
2214	2	1834	7	10	NULL	0	NULL	statement 1	Process		is dependent on					adenosine triphosphate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_279_5350_580_s_45	9438855	( D) Adenosine triphosphate-dependent MT-binding activity of Rabkinesin-6 motor domain.	bind
2855	1	1835	5	10	NULL	0	NULL	CD26	GP		bind					caveolin-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_39_14186_s_90	15353589	( D) Amino acids 201 - 211 and DPPIV of CD26 were required for binding of CD26 to caveolin-1.	bind
2856	2	1835	5	10	NULL	0	NULL	CD26	GP		is required for			amino acids 201 - 211		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_39_14186_s_90	15353589	( D) Amino acids 201 - 211 and DPPIV of CD26 were required for binding of CD26 to caveolin-1.	bind
2857	3	1835	5	10	NULL	0	NULL	CD26	GP		is required for			DPPIV		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_39_14186_s_90	15353589	( D) Amino acids 201 - 211 and DPPIV of CD26 were required for binding of CD26 to caveolin-1.	bind
2215	1	1835	7	10	NULL	0	NULL	CD26	GP		bind					caveolin-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_39_14186_s_90	15353589	( D) Amino acids 201 - 211 and DPPIV of CD26 were required for binding of CD26 to caveolin-1.	bind
2216	2	1835	7	10	NULL	0	NULL	CD26	GP		is required for			 Amino acids 201 - 211 		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_39_14186_s_90	15353589	( D) Amino acids 201 - 211 and DPPIV of CD26 were required for binding of CD26 to caveolin-1.	bind
2217	3	1835	7	10	NULL	0	NULL	CD26	GP		is required for			DPPIV 		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_39_14186_s_90	15353589	( D) Amino acids 201 - 211 and DPPIV of CD26 were required for binding of CD26 to caveolin-1.	bind
2858	1	1836	5	10	NULL	0	NULL	Mot1	GP		bind					TBPc-DNA complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_7_1492_s_70	16541100	( D) An isotherm calculated from (C) for the binding of Mot1 to the TBPc-DNA complex.	bind
2218	1	1836	7	10	NULL	0	NULL	Mot1	GP		bind					TBPc-DNA complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_7_1492_s_70	16541100	( D) An isotherm calculated from (C) for the binding of Mot1 to the TBPc-DNA complex.	bind
2859	1	1838	5	10	NULL	0	NULL	HCV	Organism		bind					CD81	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_science_282_5390_938_s_83	9794763	( D) Antibodies that neutralize HCV infection in vivo inhibit binding of HCV to CD81 in vitro.	bind
2860	2	1838	5	10	NULL	0	NULL	antibodies	GP		neutralize					HCV infection	Organism				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_science_282_5390_938_s_83	9794763	( D) Antibodies that neutralize HCV infection in vivo inhibit binding of HCV to CD81 in vitro.	bind
2861	3	1838	5	10	NULL	0	NULL	statement 2	Process		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_282_5390_938_s_83	9794763	( D) Antibodies that neutralize HCV infection in vivo inhibit binding of HCV to CD81 in vitro.	bind
2219	1	1838	7	10	NULL	0	NULL	HCV	Organism		bind					CD81	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_science_282_5390_938_s_83	9794763	( D) Antibodies that neutralize HCV infection in vivo inhibit binding of HCV to CD81 in vitro.	bind
2220	2	1838	7	10	NULL	0	NULL	Antibodies	GP		neutralize					HCV	Organism				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_science_282_5390_938_s_83	9794763	( D) Antibodies that neutralize HCV infection in vivo inhibit binding of HCV to CD81 in vitro.	bind
2222	3	1838	7	10	NULL	0	NULL	statement 2	Process		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_282_5390_938_s_83	9794763	( D) Antibodies that neutralize HCV infection in vivo inhibit binding of HCV to CD81 in vitro.	bind
2862	1	1840	5	10	NULL	0	NULL	ATP	Chemical		bind					BVR	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_20_7109_s_165	15870194	( d) ATP binding to BVR is necessary for it to phosphorylate IRS-1.	bind
2863	2	1840	5	10	NULL	0	NULL	BVR	GP		phosphorylate					IRS-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_20_7109_s_165	15870194	( d) ATP binding to BVR is necessary for it to phosphorylate IRS-1.	bind
2864	3	1840	5	10	NULL	0	NULL	statement 1	Process		is necessary for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_20_7109_s_165	15870194	( d) ATP binding to BVR is necessary for it to phosphorylate IRS-1.	bind
2223	1	1840	7	10	NULL	0	NULL	ATP	Chemical		bind					BVR	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_20_7109_s_165	15870194	( d) ATP binding to BVR is necessary for it to phosphorylate IRS-1.	bind
2224	2	1840	7	10	NULL	0	NULL	BVR 	GP		phosphorylate					IRS-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_20_7109_s_165	15870194	( d) ATP binding to BVR is necessary for it to phosphorylate IRS-1.	bind
2225	3	1840	7	10	NULL	0	NULL	statement 1	Process		is required for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_20_7109_s_165	15870194	( d) ATP binding to BVR is necessary for it to phosphorylate IRS-1.	bind
2865	1	1841	5	10	NULL	0	NULL	ATP-agarose	Chemical		bind					TAP1	GP				NULL	HeLa-M cell transfectants	NULL	NULL	NULL	NULL	gw60_embo_20_3_387_s_214	11157746	( D) ATP-agarose binding of TAP1 in the HeLa-M cell transfectants.	bind
2226	1	1841	7	10	NULL	0	NULL	ATP-agarose	Chemical		bind					TAP1	GP				NULL	in HeLa-M cell transfectants	NULL	NULL	NULL	NULL	gw60_embo_20_3_387_s_214	11157746	( D) ATP-agarose binding of TAP1 in the HeLa-M cell transfectants.	bind
2867	1	1843	5	10	NULL	0	NULL	3H-PIP2	GP		bind					GST-RKC	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_10_5820_s_76	10318968	( D) Binding of 3H-PIP2 to GST-RKC (100 nM) in the absence of antibody (control,  ), in the presence of 1 muM ( ) or 10 muM ( ) antibody (labeled Ab).	bind
2228	1	1843	7	10	NULL	0	NULL	3H-PIP2	GP		bind					GST-RKC	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_10_5820_s_76	10318968	( D) Binding of 3H-PIP2 to GST-RKC (100 nM) in the absence of antibody (control,  ), in the presence of 1 muM ( ) or 10 muM ( ) antibody (labeled Ab).	bind
2868	1	1844	5	10	NULL	0	NULL	3R-tau	GP		bind					tubulin	GP	normal			NULL		NULL	NULL	NULL	NULL	gw70_embo_22_1_70_s_72	12505985	( D) Binding of 3R-tau to normal tubulin in the absence or presence of kinesin motor  domains (K).	bind
2251	1	1844	7	10	NULL	0	NULL	3R-tau	GP		bind					tubulin	GP	normal			NULL		NULL	NULL	NULL	NULL	gw70_embo_22_1_70_s_72	12505985	( D) Binding of 3R-tau to normal tubulin in the absence or presence of kinesin motor  domains (K).	bind
2871	1	1846	5	10	NULL	0	NULL	ABI1	GP		bind					PA	GP				NULL	in vesicles	NULL	NULL	NULL	NULL	gw70_pnas_101_25_9508_s_175	15197253	( D) Binding of ABI1 and mutant proteins to PA in vesicles.	bind
2872	2	1846	5	10	NULL	0	NULL	mutant proteins	GP		bind					PA	GP				NULL	in vesicles	NULL	NULL	NULL	NULL	gw70_pnas_101_25_9508_s_175	15197253	( D) Binding of ABI1 and mutant proteins to PA in vesicles.	bind
2252	1	1846	7	10	NULL	0	NULL	ABI1	GP		bind					PA 	GP				NULL	in vesicles	NULL	NULL	NULL	NULL	gw70_pnas_101_25_9508_s_175	15197253	( D) Binding of ABI1 and mutant proteins to PA in vesicles.	bind
2253	2	1846	7	10	NULL	0	NULL	mutant proteins	GP		bind					 PA	GP				NULL	in vesicles	NULL	NULL	NULL	NULL	gw70_pnas_101_25_9508_s_175	15197253	( D) Binding of ABI1 and mutant proteins to PA in vesicles.	bind
2873	1	1847	5	10	NULL	0	NULL	biotin-GA	GP		bind					TfR	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_34_12095_s_134	16103367	( D) Binding of biotin-GA and tritium-GA to TfR is not inhibited by either apo-transferrin  or holo-transferrin.	bind
2874	2	1847	5	10	NULL	0	NULL	tritium-GA	GP		bind					TfR	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_34_12095_s_134	16103367	( D) Binding of biotin-GA and tritium-GA to TfR is not inhibited by either apo-transferrin  or holo-transferrin.	bind
2875	3	1847	5	10	NULL	0	NULL	statement 1	Process		is not inhibited by					apo-transferrin	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_34_12095_s_134	16103367	( D) Binding of biotin-GA and tritium-GA to TfR is not inhibited by either apo-transferrin  or holo-transferrin.	bind
2876	4	1847	5	10	NULL	0	NULL	statement 2	Process		is not inhibited by					apo-transferrin	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_34_12095_s_134	16103367	( D) Binding of biotin-GA and tritium-GA to TfR is not inhibited by either apo-transferrin  or holo-transferrin.	bind
2877	5	1847	5	10	NULL	0	NULL	statement 1	Process		is not inhibited by					holo-transferrin	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_34_12095_s_134	16103367	( D) Binding of biotin-GA and tritium-GA to TfR is not inhibited by either apo-transferrin  or holo-transferrin.	bind
2878	6	1847	5	10	NULL	0	NULL	statement 2	Process		is not inhibited by					holo-transferrin	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_34_12095_s_134	16103367	( D) Binding of biotin-GA and tritium-GA to TfR is not inhibited by either apo-transferrin  or holo-transferrin.	bind
2254	1	1847	7	10	NULL	0	NULL	biotin-GA	GP		bind					TfR	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_34_12095_s_134	16103367	( D) Binding of biotin-GA and tritium-GA to TfR is not inhibited by either apo-transferrin  or holo-transferrin.	bind
2255	2	1847	7	10	NULL	0	NULL	tritium-GA	GP		bind					TfR	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_34_12095_s_134	16103367	( D) Binding of biotin-GA and tritium-GA to TfR is not inhibited by either apo-transferrin  or holo-transferrin.	bind
2256	3	1847	7	10	NULL	0	NULL	statement 1	Process		is not inhibited by					apo-transferrin	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_34_12095_s_134	16103367	( D) Binding of biotin-GA and tritium-GA to TfR is not inhibited by either apo-transferrin  or holo-transferrin.	bind
2257	4	1847	7	10	NULL	0	NULL	statement 1	Process		is not inhibited by					holo-transferrin	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_34_12095_s_134	16103367	( D) Binding of biotin-GA and tritium-GA to TfR is not inhibited by either apo-transferrin  or holo-transferrin.	bind
2258	5	1847	7	10	NULL	0	NULL	statement 2	Process		is not inhibited by					apo-transferrin	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_34_12095_s_134	16103367	( D) Binding of biotin-GA and tritium-GA to TfR is not inhibited by either apo-transferrin  or holo-transferrin.	bind
2259	6	1847	7	10	NULL	0	NULL	statement 2	Process		is not inhibited by					holo-transferrin	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_34_12095_s_134	16103367	( D) Binding of biotin-GA and tritium-GA to TfR is not inhibited by either apo-transferrin  or holo-transferrin.	bind
2879	1	1848	5	10	NULL	0	NULL	BRCA1	GP		bind					CBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_3_1020_s_161	10655477	( D) Binding of BRCA1 to CBP is not affected by phosphorylation.	bind
2880	2	1848	5	10	NULL	0	NULL	statement 1	Process		is not affected by					phosphorylation	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_3_1020_s_161	10655477	( D) Binding of BRCA1 to CBP is not affected by phosphorylation.	bind
2260	1	1848	7	10	NULL	0	NULL	BRCA1	GP		bind					CBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_3_1020_s_161	10655477	( D) Binding of BRCA1 to CBP is not affected by phosphorylation.	bind
2261	2	1848	7	10	NULL	0	NULL	statement 1	Process		is not affected by 					phosphorylation	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_3_1020_s_161	10655477	( D) Binding of BRCA1 to CBP is not affected by phosphorylation.	bind
2881	1	1849	5	10	NULL	0	NULL				bind			CBD		collagen	GP	insoluble			NULL		NULL	NULL	NULL	NULL	gw60_embo_22_8_1743_s_140	12682007	( D) Binding of CBD to insoluble collagen.	bind
2262	1	1849	7	10	NULL	0	NULL				bind			CBD		collagen	GP	insoluble			NULL		NULL	NULL	NULL	NULL	gw60_embo_22_8_1743_s_140	12682007	( D) Binding of CBD to insoluble collagen.	bind
2882	1	1850	5	10	NULL	0	NULL	Chordin	GP		bind					Bmp2	GP	Cvl2-N saturated;; immobilized			NULL		NULL	NULL	NULL	NULL	gw70_development_133_5_801_s_203	16439480	( D) Binding of Chordin to Cvl2-N saturated immobilized Bmp2.	bind
2263	1	1850	7	10	NULL	0	NULL	Chordin	GP		bind					Bmp2	GP	Cvl2-N saturated;; immobilized			NULL		NULL	NULL	NULL	NULL	gw70_development_133_5_801_s_203	16439480	( D) Binding of Chordin to Cvl2-N saturated immobilized Bmp2.	bind
2901	1	1851	5	10	NULL	0	NULL	CNTF	GP		activate					STAT1	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_278_5337_477_s_168	9334309	( D) Binding of CNTF-activated STAT1 and STAT3 to a specific site within the GFAP promoter ( 47).	bind
2902	2	1851	5	10	NULL	0	NULL	CNTF	GP		activate					STAT3	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_278_5337_477_s_168	9334309	( D) Binding of CNTF-activated STAT1 and STAT3 to a specific site within the GFAP promoter ( 47).	bind
2903	3	1851	5	10	NULL	0	NULL	statement 1	Process		bind					GFAP	GP			a specific site within promoter	NULL		NULL	NULL	NULL	NULL	gw60_science_278_5337_477_s_168	9334309	( D) Binding of CNTF-activated STAT1 and STAT3 to a specific site within the GFAP promoter ( 47).	bind
2904	4	1851	5	10	NULL	0	NULL	statement 2	Process		bind					GFAP	GP			a specific site within promoter	NULL		NULL	NULL	NULL	NULL	gw60_science_278_5337_477_s_168	9334309	( D) Binding of CNTF-activated STAT1 and STAT3 to a specific site within the GFAP promoter ( 47).	bind
2264	1	1851	7	10	NULL	0	NULL	CNTF	GP		activate					STAT1	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_278_5337_477_s_168	9334309	( D) Binding of CNTF-activated STAT1 and STAT3 to a specific site within the GFAP promoter ( 47).	bind
2265	2	1851	7	10	NULL	0	NULL	CNTF	GP		activate					STAT3	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_278_5337_477_s_168	9334309	( D) Binding of CNTF-activated STAT1 and STAT3 to a specific site within the GFAP promoter ( 47).	bind
3446	3	1851	7	10	NULL	0	NULL	statement 1	Process		bind					GFAP	GP			specific site within the promoter of 	NULL		NULL	NULL	NULL	NULL	gw60_science_278_5337_477_s_168	9334309	( D) Binding of CNTF-activated STAT1 and STAT3 to a specific site within the GFAP promoter ( 47).	bind
3447	4	1851	7	10	NULL	0	NULL	statement 2	GP		bind					GFAP	GP			specific site within the promoter of 	NULL		NULL	NULL	NULL	NULL	gw60_science_278_5337_477_s_168	9334309	( D) Binding of CNTF-activated STAT1 and STAT3 to a specific site within the GFAP promoter ( 47).	bind
2905	1	1852	5	10	NULL	0	NULL	His6-C-mu2	GP		bind					PIPK Igamma kinase	GP		core domain		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_32_11934_s_99	16880396	( D) Binding of His6-C-mu2 to the PIPK Igamma kinase core domain determined by surface plasmon resonance.	bind
2266	1	1852	7	10	NULL	0	NULL	His6-C-mu2	GP		binds to					PIPK Igamma kinase 	GP		core domain		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_32_11934_s_99	16880396	( D) Binding of His6-C-mu2 to the PIPK Igamma kinase core domain determined by surface plasmon resonance.	bind
2906	1	1853	5	10	NULL	0	NULL	JNK	GP		bind					NFAT4	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_278_5343_1638_s_52	9374467	( D) Binding of JNK and calcineurin to different sites on NFAT4.	bind
2907	2	1853	5	10	NULL	0	NULL	calcineurin	GP		bind					NFAT4	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_278_5343_1638_s_52	9374467	( D) Binding of JNK and calcineurin to different sites on NFAT4.	bind
2267	1	1853	7	10	NULL	0	NULL	JNK	GP		bind					NFAT4	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_278_5343_1638_s_52	9374467	( D) Binding of JNK and calcineurin to different sites on NFAT4.	bind
2268	2	1853	7	10	NULL	0	NULL	calcineurin	GP		bind					NFAT4	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_278_5343_1638_s_52	9374467	( D) Binding of JNK and calcineurin to different sites on NFAT4.	bind
3071	1	1854	5	10	NULL	0	NULL	JNK1	GP		bind					JIP-1	GP	deletion mutant	residues between127-202		NULL		NULL	NULL	NULL	NULL	gw60_science_277_5326_693_s_42	9235893	( D) Binding of JNK1 and JNK2 to GST and GST fusion proteins corresponding to JIP-1 with small deletions between residues 127 and 202.	bind
3072	2	1854	5	10	NULL	0	NULL	JNK2	GP		bind					JIP-1	GP	deletion mutant	residues between 127-202		NULL		NULL	NULL	NULL	NULL	gw60_science_277_5326_693_s_42	9235893	( D) Binding of JNK1 and JNK2 to GST and GST fusion proteins corresponding to JIP-1 with small deletions between residues 127 and 202.	bind
2270	1	1854	7	10	NULL	0	NULL	JNK1 	GP		bind					JIP-1	GP	deletion mutant	between residues 127 and 202		NULL		NULL	NULL	NULL	NULL	gw60_science_277_5326_693_s_42	9235893	( D) Binding of JNK1 and JNK2 to GST and GST fusion proteins corresponding to JIP-1 with small deletions between residues 127 and 202.	bind
2272	2	1854	7	10	NULL	0	NULL	JNK2	GP		bind					JIP-1	GP	deletion mutant	between residues 127 and 202		NULL		NULL	NULL	NULL	NULL	gw60_science_277_5326_693_s_42	9235893	( D) Binding of JNK1 and JNK2 to GST and GST fusion proteins corresponding to JIP-1 with small deletions between residues 127 and 202.	bind
2908	1	1855	5	10	NULL	0	NULL	myostatin	GP 		bind					ActRIIB	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_16_9306_s_63	11459935	( d) Binding of myostatin to ActRIIB.	bind
2273	1	1855	7	10	NULL	0	NULL	myostatin	GP		bind					ActRIIB	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_16_9306_s_63	11459935	( d) Binding of myostatin to ActRIIB.	bind
2928	1	1856	5	10	NULL	0	NULL	NC	GP		bind									(TG)4	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_2_472_s_118	16434700	( D) Binding of NC to (TG)4 in buffer containing 250 mM rather than 150 mM NaCl.	bind
2274	1	1856	7	10	NULL	0	NULL	NC	GP		bind									(TG)4	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_2_472_s_118	16434700	( D) Binding of NC to (TG)4 in buffer containing 250 mM rather than 150 mM NaCl.	bind
2912	1	1857	5	10	NULL	0	NULL	NFAT family members	GP		bind					Sp1	GP				NULL	NHK cells exposed to high Ca2+	NULL	NULL	NULL	NULL	gw70_pnas_102_39_13921_s_48	16172401	( d) Binding of NFAT family members to Sp1 on exposure of NHK cells to high Ca2+.	bind
2275	1	1857	7	10	NULL	0	NULL	NFAT family	GP		bind					Sp1	GP				NULL	in NHK cells exposed to high Ca2+	NULL	NULL	NULL	NULL	gw70_pnas_102_39_13921_s_48	16172401	( d) Binding of NFAT family members to Sp1 on exposure of NHK cells to high Ca2+.	bind
2919	1	1859	5	10	NULL	0	NULL	Sho1	GP		bind					Ste50	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_13_3033_s_48	16778768	( D) Binding of Sho1 to Ste50 and Ste11.	bind
2920	2	1859	5	10	NULL	0	NULL	Sho1	GP		bind					Ste11	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_13_3033_s_48	16778768	( D) Binding of Sho1 to Ste50 and Ste11.	bind
2277	1	1859	7	10	NULL	0	NULL	Sho1	GP		bind					Ste50	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_13_3033_s_48	16778768	( D) Binding of Sho1 to Ste50 and Ste11.	bind
2278	2	1859	7	10	NULL	0	NULL	Sho1	GP		bind					Ste11	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_13_3033_s_48	16778768	( D) Binding of Sho1 to Ste50 and Ste11.	bind
2921	1	1860	5	10	NULL	0	NULL	FGF-7	GP	soluble	bind					perlecan	Chemical	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_8_1599_s_187	9788974	( D) Binding of soluble FGF-7 to  immobilized perlecan (4 mug) in the presence of increasing concentrations of heparan sulfate as indicated.	bind
2923	2	1860	5	10	NULL	0	NULL	statement 1	Process		in the presence of					heparan sulfate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_8_1599_s_187	9788974	( D) Binding of soluble FGF-7 to  immobilized perlecan (4 mug) in the presence of increasing concentrations of heparan sulfate as indicated.	bind
2279	1	1860	7	10	NULL	0	NULL	FGF-7	GP	soluble	bind					perlecan	Chemical	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_8_1599_s_187	9788974	( D) Binding of soluble FGF-7 to  immobilized perlecan (4 mug) in the presence of increasing concentrations of heparan sulfate as indicated.	bind
46207	2	1860	7	10	NULL	0	NULL	statement 1	Process		in presence of					heparan sulfate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_8_1599_s_187	9788974	( D) Binding of soluble FGF-7 to  immobilized perlecan (4 mug) in the presence of increasing concentrations of heparan sulfate as indicated.	bind
2933	1	1861	5	10	NULL	0	NULL	RBP-Jkappa protein	GP		bind					p21	GP	endogenous		promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_20_13_3427_s_139	11432830	( D) Binding of the RBP-Jkappa protein to the endogenous p21 promoter as assessed by chromatin immunoprecipitation.	bind
2280	1	1861	7	10	NULL	0	NULL	RBP-Jkappa protein	GP		bind					p21	GP	endogenous		promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_20_13_3427_s_139	11432830	( D) Binding of the RBP-Jkappa protein to the endogenous p21 promoter as assessed by chromatin immunoprecipitation.	bind
2937	1	1862	5	10	NULL	0	NULL	ubiquitin chains	GP		bind					Vps9	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_6_1273_s_116	12628920	( D) Binding of ubiquitin chains to Vps9 and Cue1 CUE domains.	bind
2939	2	1862	5	10	NULL	0	NULL	ubiquitin chains	GP		bind					Cue1	GP		CUE domains		NULL		NULL	NULL	NULL	NULL	gw60_embo_22_6_1273_s_116	12628920	( D) Binding of ubiquitin chains to Vps9 and Cue1 CUE domains.	bind
2281	1	1862	7	10	NULL	0	NULL	ubiquitin chains	GP		bind					Vps9	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_6_1273_s_116	12628920	( D) Binding of ubiquitin chains to Vps9 and Cue1 CUE domains.	bind
2282	2	1862	7	10	NULL	0	NULL	ubiquitin chains	GP		bind					Cue1	GP		CUE		NULL		NULL	NULL	NULL	NULL	gw60_embo_22_6_1273_s_116	12628920	( D) Binding of ubiquitin chains to Vps9 and Cue1 CUE domains.	bind
2943	1	1863	5	10	NULL	0	NULL	GST-KAPP fusion protein	GP	truncated	bind					MBP fusions	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_14_7821_s_119	10393905	( D) Binding results between truncated GST-KAPP fusion proteins and MBP fusions.	bind
2283	1	1863	7	10	NULL	0	NULL	GST-KAPP fusion proteins	GP	truncated	bind					MBP fusions	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_14_7821_s_119	10393905	( D) Binding results between truncated GST-KAPP fusion proteins and MBP fusions.	bind
2947	1	1864	5	10	NULL	0	NULL	BRG1	GP		associate with					chromatin	Chromosome	downstream			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_11_1392_s_138	12782657	( D) BRG1 association with downstream  chromatin following heat shock depends on polymerase movement.	bind
2948	2	1864	5	10	NULL	0	NULL	statement 1	Process		occurs following					heat shock	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_11_1392_s_138	12782657	( D) BRG1 association with downstream  chromatin following heat shock depends on polymerase movement.	bind
2950	3	1864	5	10	NULL	0	NULL	statement 1	Process		depends on					polymerase	GP	movement of			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_11_1392_s_138	12782657	( D) BRG1 association with downstream  chromatin following heat shock depends on polymerase movement.	bind
2284	1	1864	7	10	NULL	0	NULL	BRG1	GP		bind					chromatin	Chromosome	downstream			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_11_1392_s_138	12782657	( D) BRG1 association with downstream  chromatin following heat shock depends on polymerase movement.	bind
2285	2	1864	7	10	NULL	0	NULL	statement 1	Process		occurs upon					heat shock 	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_11_1392_s_138	12782657	( D) BRG1 association with downstream  chromatin following heat shock depends on polymerase movement.	bind
2286	3	1864	7	10	NULL	0	NULL	statement 1	Process		depends on					polymerase	GP	movement of			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_11_1392_s_138	12782657	( D) BRG1 association with downstream  chromatin following heat shock depends on polymerase movement.	bind
2951	1	1865	5	10	NULL	0	NULL	C-Maf	GP		bind					IL-4	GP			promoter DNA	NULL		NULL	NULL	NULL	NULL	gw60_embo_18_2_420_s_189	9889198	( D) C-Maf binding to IL-4 promoter DNA is facilitated by phosphorylated JunB.	bind
2953	2	1865	5	10	NULL	0	NULL	statement 1	Process		is facilitated by					JunB	GP	phosphorylated			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_2_420_s_189	9889198	( D) C-Maf binding to IL-4 promoter DNA is facilitated by phosphorylated JunB.	bind
2287	1	1865	7	10	NULL	0	NULL	C-Maf	GP		bind					IL-4	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_18_2_420_s_189	9889198	( D) C-Maf binding to IL-4 promoter DNA is facilitated by phosphorylated JunB.	bind
2288	2	1865	7	10	NULL	0	NULL	statement 1	Process		is facilitated by 					JunB	GP	phosphorylated			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_2_420_s_189	9889198	( D) C-Maf binding to IL-4 promoter DNA is facilitated by phosphorylated JunB.	bind
2954	1	1866	5	10	NULL	0	NULL	c-Myc	GP		bind		directly			bmi-1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_10_3645_s_67	16537449	( D) c-Myc binds directly to the  bmi-1 promoter.	bind
2289	1	1866	7	10	NULL	0	NULL	c-Myc	GP		bind		directly			bmi-1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_10_3645_s_67	16537449	( D) c-Myc binds directly to the  bmi-1 promoter.	bind
2955	1	1867	5	10	NULL	0	NULL	TR	GP		bind					E1A	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_18_6267_s_84	15849266	( D) CBM peptide blocks TR binding to E1A and N-CoR.	bind
2956	2	1867	5	10	NULL	0	NULL	TR	GP		bind					N-CoR	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_18_6267_s_84	15849266	( D) CBM peptide blocks TR binding to E1A and N-CoR.	bind
2957	3	1867	5	10	NULL	0	NULL	CBM peptide	GP		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_18_6267_s_84	15849266	( D) CBM peptide blocks TR binding to E1A and N-CoR.	bind
2958	4	1867	5	10	NULL	0	NULL	CBM peptide	GP		blocks					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_18_6267_s_84	15849266	( D) CBM peptide blocks TR binding to E1A and N-CoR.	bind
2290	1	1867	7	10	NULL	0	NULL	TR	GP		bind					E1A	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_18_6267_s_84	15849266	( D) CBM peptide blocks TR binding to E1A and N-CoR.	bind
2291	2	1867	7	10	NULL	0	NULL	TR	GP		bind					N-CoR	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_18_6267_s_84	15849266	( D) CBM peptide blocks TR binding to E1A and N-CoR.	bind
2292	3	1867	7	10	NULL	0	NULL	CBM peptide	GP		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_18_6267_s_84	15849266	( D) CBM peptide blocks TR binding to E1A and N-CoR.	bind
2293	4	1867	7	10	NULL	0	NULL	CBM peptide	GP		blocks					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_18_6267_s_84	15849266	( D) CBM peptide blocks TR binding to E1A and N-CoR.	bind
2959	1	1868	5	10	NULL	0	NULL	CCT	GP		bind					Gbeta	GP		WD40 repeats		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_22_8360_s_95	16717193	( D) CCT binding to individual WD40 repeats of Gbeta ( n = 3).	bind
2294	1	1868	7	10	NULL	0	NULL	CCT	GP		bind					Gbeta	GP		WD40 repeats		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_22_8360_s_95	16717193	( D) CCT binding to individual WD40 repeats of Gbeta ( n = 3).	bind
2960	1	1869	5	10	NULL	0	NULL	p27	GP		bind					Cdk2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_104_7_865_s_111	10510327	( d) Cdk2 immunoprecipitates: p27 bound to Cdk2, Cdk2 level, and Cdk2 activity in total (left column) or fractionated extracts (remaining columns).	bind
2295	1	1869	7	10	NULL	0	NULL	 p27 	GP		bind					Cdk2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_104_7_865_s_111	10510327	( d) Cdk2 immunoprecipitates: p27 bound to Cdk2, Cdk2 level, and Cdk2 activity in total (left column) or fractionated extracts (remaining columns).	bind
2965	1	1872	5	10	NULL	0	NULL	SRF	GP		bind							endogenous		CArG regions	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_16_5271_s_415	16170155	( D) ChIP analysis of SRF binding to the endogenous CArG regions.	bind
2296	1	1872	7	10	NULL	0	NULL	SRF	GP		bind							endogenous		CArG regions	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_16_5271_s_415	16170155	( D) ChIP analysis of SRF binding to the endogenous CArG regions.	bind
2966	1	1873	5	10	NULL	0	NULL	E6	GP		bind					hTERT	GP	endogenous		promoter	NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_14_8211_s_185	12821782	( D) CHIP assay detects E6 and Myc proteins  bound to the endogenous hTERT promoter.	bind
2967	2	1873	5	10	NULL	0	NULL	Myc proteins	GP		bind					hTERT	GP	endogenous		promoter	NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_14_8211_s_185	12821782	( D) CHIP assay detects E6 and Myc proteins  bound to the endogenous hTERT promoter.	bind
2297	1	1873	7	10	NULL	0	NULL	E6	GP		bind					hTERT	GP	endogenous		promoter	NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_14_8211_s_185	12821782	( D) CHIP assay detects E6 and Myc proteins  bound to the endogenous hTERT promoter.	bind
2298	2	1873	7	10	NULL	0	NULL	Myc	GP		bind					hTERT	GP	endogenous		promoter	NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_14_8211_s_185	12821782	( D) CHIP assay detects E6 and Myc proteins  bound to the endogenous hTERT promoter.	bind
3284	1	1874	7	10	NULL	0	NULL	Nfatc3	NULL		binds	NULL				Sftpb	NULL			 5''-regulatory region	NULL	MLE-15 cells 	NULL	NULL	NULL	NULL	gw70_jclininvest_116_10_2597_s_128	16998587	( D) ChIP assays on 5''-regulatory regions of  Sftpb and  Abca3 gene (black boxes, GGAAA; white boxes, AGAAA) in MLE-15 cells, which express high  levels of Nfatc3 identified direct binding of Nfatc3 in the chromatin.	bind
3285	2	1874	7	NULL	NULL	0	NULL	Nfatc3	NULL		binds	NULL				Abca3	NULL			5''-regulatory region	NULL	MLE-15 cells	NULL	NULL	NULL	NULL	gw70_jclininvest_116_10_2597_s_128	16998587	( D) ChIP assays on 5''-regulatory regions of  Sftpb and  Abca3 gene (black boxes, GGAAA; white boxes, AGAAA) in MLE-15 cells, which express high  levels of Nfatc3 identified direct binding of Nfatc3 in the chromatin.	bind
3445	3	1874	7	NULL	NULL	0	NULL	MLE-15 cells	NULL		express	NULL				Nfatc3 	NULL	high levels of 			NULL		0	NULL	NULL	NULL	gw70_jclininvest_116_10_2597_s_128	16998587	( D) ChIP assays on 5''-regulatory regions of  Sftpb and  Abca3 gene (black boxes, GGAAA; white boxes, AGAAA) in MLE-15 cells, which express high  levels of Nfatc3 identified direct binding of Nfatc3 in the chromatin.	bind
2970	1	1875	5	10	NULL	0	NULL	Chk1	GP		bind					PPM1D	GP	mutant forms			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_10_1162_s_86	15870257	( D) Chk1 binds to mutant forms of PPM1D except for one mutant missing part of the phosphatase  domain.	bind
2971	2	1875	5	10	NULL	0	NULL	Chk1	GP		does not bind					PPM1D	GP	mutant missing part of	phosphatase domain		NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_10_1162_s_86	15870257	( D) Chk1 binds to mutant forms of PPM1D except for one mutant missing part of the phosphatase  domain.	bind
2330	1	1875	7	10	NULL	0	NULL	Chk1	GP		bind					PPM1D	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_10_1162_s_86	15870257	( D) Chk1 binds to mutant forms of PPM1D except for one mutant missing part of the phosphatase  domain.	bind
2331	2	1875	7	10	NULL	0	NULL	Chk1	GP		does not bind					PPM1D	GP	mutant missing part of  	phosphatase domain		NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_10_1162_s_86	15870257	( D) Chk1 binds to mutant forms of PPM1D except for one mutant missing part of the phosphatase  domain.	bind
2972	1	1876	5	10	NULL	0	NULL	EWS - WT1(+KTS)	GP		bind									HC63	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_genesdev_17_17_2094_s_90	12923058	( D) Chromatin immunoprecipitation (ChIP) analysis to demonstrate in  vivo binding of  EWS - WT1(+KTS) to HC63.	bind
2332	1	1876	7	10	NULL	0	NULL	EWS - WT1(+KTS)	GP		bind									HC63	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_genesdev_17_17_2094_s_90	12923058	( D) Chromatin immunoprecipitation (ChIP) analysis to demonstrate in  vivo binding of  EWS - WT1(+KTS) to HC63.	bind
2973	1	1877	5	10	NULL	0	NULL	Gdf11	GP		bind					IIA	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_21_2749_s_117	12414726	( D) Coimmunoprecipitation analyses showing that Gdf11 binds to IIA and IIB to different degrees.	bind
2974	2	1877	5	10	NULL	0	NULL	Gdf11	GP		bind					IIB	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_21_2749_s_117	12414726	( D) Coimmunoprecipitation analyses showing that Gdf11 binds to IIA and IIB to different degrees.	bind
2333	1	1877	7	10	NULL	0	NULL	Gdf11	GP		bind					IIA	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_21_2749_s_117	12414726	( D) Coimmunoprecipitation analyses showing that Gdf11 binds to IIA and IIB to different degrees.	bind
2334	2	1877	7	10	NULL	0	NULL	Gdf11	GP		bind					IIB	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_21_2749_s_117	12414726	( D) Coimmunoprecipitation analyses showing that Gdf11 binds to IIA and IIB to different degrees.	bind
2975	1	1878	5	10	NULL	0	NULL	kinesin	GP		bind					CPEB-myc13	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_5_638_s_131	12629046	( D) Coimmunoprecipitation of kinesin and dynein with CPEB-myc13.	bind
2976	2	1878	5	10	NULL	0	NULL	dynein	GP		bind					CPEB-myc13	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_5_638_s_131	12629046	( D) Coimmunoprecipitation of kinesin and dynein with CPEB-myc13.	bind
2335	1	1878	7	10	NULL	NULL	NULL	kinesin	GP		 bind					CPEB-myc13	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_5_638_s_131	12629046	( D) Coimmunoprecipitation of kinesin and dynein with CPEB-myc13.	bind
2336	2	1878	7	10	NULL	NULL	NULL	dynein 	GP		bind					CPEB-myc13	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_5_638_s_131	12629046	( D) Coimmunoprecipitation of kinesin and dynein with CPEB-myc13.	bind
2977	1	1879	5	10	NULL	NULL	NULL	c-Myb	GP		bind					GST-histone H3	GP		tail		NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_20_2447_s_63	16195416	( D) Comparison of c-Myb binding to various GST-histone H3 tail constructs.	bind
2337	1	1879	7	10	NULL	NULL	NULL	c-Myb	GP		bind					GST-histone H3	GP		tail		NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_20_2447_s_63	16195416	( D) Comparison of c-Myb binding to various GST-histone H3 tail constructs.	bind
2978	1	1880	5	10	NULL	NULL	NULL	CD-40-p1	GP		bind					TRAF2	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_15_8408_s_151	10411888	( D) Comparison of CD-40-p1 (orange) and TNF-R2 (light blue) bound to TRAF2 (CD40-p1 complex, gray; TNF-R2 complex, blue).	bind
2979	2	1880	5	10	NULL	NULL	NULL	TNF-R2	GP		bind					TRAF2	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_15_8408_s_151	10411888	( D) Comparison of CD-40-p1 (orange) and TNF-R2 (light blue) bound to TRAF2 (CD40-p1 complex, gray; TNF-R2 complex, blue).	bind
2338	1	1880	7	10	NULL	NULL	NULL	CD-40-p1	GP		bind					TRAF2	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_15_8408_s_151	10411888	( D) Comparison of CD-40-p1 (orange) and TNF-R2 (light blue) bound to TRAF2 (CD40-p1 complex, gray; TNF-R2 complex, blue).	bind
2339	2	1880	7	10	NULL	NULL	NULL	TNF-R2	GP		bind					TRAF2	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_15_8408_s_151	10411888	( D) Comparison of CD-40-p1 (orange) and TNF-R2 (light blue) bound to TRAF2 (CD40-p1 complex, gray; TNF-R2 complex, blue).	bind
2980	1	1881	5	10	NULL	NULL	NULL	malonyl-CoA	Chemical		bind					CPT1a	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_19_7282_s_56	16651524	( D) Comparison of malonyl-CoA binding to CPT1a and CPT1c.	bind
2981	2	1881	5	10	NULL	NULL	NULL	malonyl-CoA	Chemical		bind					CPT1c	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_19_7282_s_56	16651524	( D) Comparison of malonyl-CoA binding to CPT1a and CPT1c.	bind
2340	1	1881	7	10	NULL	NULL	NULL	malonyl-CoA	Chemical		bind					CPT1a	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_19_7282_s_56	16651524	( D) Comparison of malonyl-CoA binding to CPT1a and CPT1c.	bind
2341	2	1881	7	10	NULL	NULL	NULL	malonyl-CoA	Chemical		bind					CPT1c	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_19_7282_s_56	16651524	( D) Comparison of malonyl-CoA binding to CPT1a and CPT1c.	bind
2982	1	1882	5	10	NULL	NULL	NULL	RBD12	GP	nucleolin 	bind					b2	GP			NRE	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_22_6461_s_73	14602904	( D) Competition experiments of nucleolin RBD12 binding to b2NRE.	bind
2342	1	1882	7	10	NULL	NULL	NULL	RBD12	GP	nucleolin	bind					b2	GP			NRE	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_22_6461_s_73	14602904	( D) Competition experiments of nucleolin RBD12 binding to b2NRE.	bind
2983	1	1883	5	10	NULL	NULL	NULL	TNP-ATP	Chemical		bind					Kir6.2 proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_7_1318_s_37	15775962	( D) Competition of 10 muM TNP-ATP binding to Kir6.2 proteins by PIP2.	bind
2984	2	1883	5	10	NULL	NULL	NULL	PIP2	Chemical		bind					Kir6.2 proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_7_1318_s_37	15775962	( D) Competition of 10 muM TNP-ATP binding to Kir6.2 proteins by PIP2.	bind
3282	3	1883	5	10	NULL	NULL	NULL	statement 1	Process		compete with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_7_1318_s_37	15775962	( D) Competition of 10 muM TNP-ATP binding to Kir6.2 proteins by PIP2.	bind
2344	1	1883	7	10	NULL	NULL	NULL	TNP-ATP	Chemical		bind					Kir6.2	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_7_1318_s_37	15775962	( D) Competition of 10 muM TNP-ATP binding to Kir6.2 proteins by PIP2.	bind
2345	2	1883	7	10	NULL	NULL	NULL	PIP2	Chemical		bind					Kir6.2	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_7_1318_s_37	15775962	( D) Competition of 10 muM TNP-ATP binding to Kir6.2 proteins by PIP2.	bind
4224	3	1883	7	10	NULL	NULL	NULL	statement 1	Process		compete with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_7_1318_s_37	15775962	( D) Competition of 10 muM TNP-ATP binding to Kir6.2 proteins by PIP2.	bind
2985	1	1884	5	10	NULL	NULL	NULL	Fab 2F1	GP		bind					G9-280-HLA-A2 complexes	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_14_9421_s_87	12093904	( D) Competition of MHC-peptide complexes for binding of Fab 2F1 to immobolized G9-280-HLA-A2 complexes; W/O, without competitior.	bind
2986	2	1884	5	10	NULL	NULL	NULL	MHC-peptide complexes	GP		bind					G9-280-HLA-A2 complexes	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_14_9421_s_87	12093904	( D) Competition of MHC-peptide complexes for binding of Fab 2F1 to immobolized G9-280-HLA-A2 complexes; W/O, without competitior.	bind
2346	1	1884	7	10	NULL	NULL	NULL	Fab 2F1	GP		bind					G9-280-HLA-A2 complexes	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_14_9421_s_87	12093904	( D) Competition of MHC-peptide complexes for binding of Fab 2F1 to immobolized G9-280-HLA-A2 complexes; W/O, without competitior.	bind
2347	2	1884	7	10	NULL	NULL	NULL	MHC-peptide complexes	GP		bind					G9-280-HLA-A2 complexes	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_14_9421_s_87	12093904	( D) Competition of MHC-peptide complexes for binding of Fab 2F1 to immobolized G9-280-HLA-A2 complexes; W/O, without competitior.	bind
2987	1	1885	5	10	NULL	NULL	NULL	actin	GP		bind					ABD/1-24	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_21_3442_s_117	9808630	( D) Concentration-dependent binding of actin to ABD/1-24.	bind
2348	1	1885	7	10	NULL	NULL	NULL	actin	GP		bind					ABD/1-24	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_21_3442_s_117	9808630	( D) Concentration-dependent binding of actin to ABD/1-24.	bind
3008	1	1886	5	10	NULL	NULL	NULL	CHO cells	Cell		express					alphaIIbbeta3	GP	WT			NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_42	12730600	( D) Constitutive fibrinogen binding to CHO cells expressing WT alphaIIbbeta3 and the G702N and G708N beta3 mutants as a function of fibrinogen concentration.	bind
3009	2	1886	5	10	NULL	NULL	NULL	CHO cells	Cell		express					beta3	GP	mutant	G702N		NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_42	12730600	( D) Constitutive fibrinogen binding to CHO cells expressing WT alphaIIbbeta3 and the G702N and G708N beta3 mutants as a function of fibrinogen concentration.	bind
3010	3	1886	5	10	NULL	NULL	NULL	CHO cells	Cell		express					beta3	GP	mutant	G708N		NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_42	12730600	( D) Constitutive fibrinogen binding to CHO cells expressing WT alphaIIbbeta3 and the G702N and G708N beta3 mutants as a function of fibrinogen concentration.	bind
3011	4	1886	5	10	NULL	NULL	NULL	fibrinogen	GP		bind		constitutively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_42	12730600	( D) Constitutive fibrinogen binding to CHO cells expressing WT alphaIIbbeta3 and the G702N and G708N beta3 mutants as a function of fibrinogen concentration.	bind
3012	5	1886	5	10	NULL	NULL	NULL	fibrinogen	GP		bind		constitutively			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_42	12730600	( D) Constitutive fibrinogen binding to CHO cells expressing WT alphaIIbbeta3 and the G702N and G708N beta3 mutants as a function of fibrinogen concentration.	bind
3013	6	1886	5	10	NULL	NULL	NULL	fibrinogen	GP		bind		constitutively			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_42	12730600	( D) Constitutive fibrinogen binding to CHO cells expressing WT alphaIIbbeta3 and the G702N and G708N beta3 mutants as a function of fibrinogen concentration.	bind
2349	1	1886	7	10	NULL	NULL	NULL	CHO cells 	Cell		express					alphaIIbbeta3	GP	WT			NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_42	12730600	( D) Constitutive fibrinogen binding to CHO cells expressing WT alphaIIbbeta3 and the G702N and G708N beta3 mutants as a function of fibrinogen concentration.	bind
46213	2	1886	7	10	NULL	NULL	NULL	CHO cells	Cell		express					beta3	GP	mutant	G702N		NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_42	12730600	( D) Constitutive fibrinogen binding to CHO cells expressing WT alphaIIbbeta3 and the G702N and G708N beta3 mutants as a function of fibrinogen concentration.	bind
46214	3	1886	7	10	NULL	NULL	NULL	CHO cells	Cell		express					beta3	GP	mutant	G708N		NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_42	12730600	( D) Constitutive fibrinogen binding to CHO cells expressing WT alphaIIbbeta3 and the G702N and G708N beta3 mutants as a function of fibrinogen concentration.	bind
46215	4	1886	7	10	NULL	NULL	NULL	fibrinogen	GP		bind		constitutively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_42	12730600	( D) Constitutive fibrinogen binding to CHO cells expressing WT alphaIIbbeta3 and the G702N and G708N beta3 mutants as a function of fibrinogen concentration.	bind
46216	5	1886	7	10	NULL	NULL	NULL	fibrinogen	GP		bind		constitutively			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_42	12730600	( D) Constitutive fibrinogen binding to CHO cells expressing WT alphaIIbbeta3 and the G702N and G708N beta3 mutants as a function of fibrinogen concentration.	bind
46217	6	1886	7	10	NULL	NULL	NULL	fibrinogen	GP		bind		constitutively			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_42	12730600	( D) Constitutive fibrinogen binding to CHO cells expressing WT alphaIIbbeta3 and the G702N and G708N beta3 mutants as a function of fibrinogen concentration.	bind
2989	1	1887	5	10	NULL	NULL	NULL	CREB	GP		bind					nNOS	GP			CREs	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_15_8617_s_165	10900019	( D) CREB and ATF-2 bind to the nNOS CREs.	bind
2990	2	1887	5	10	NULL	NULL	NULL	ATF-2	GP		bind					nNOS	GP			CREs	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_15_8617_s_165	10900019	( D) CREB and ATF-2 bind to the nNOS CREs.	bind
2351	1	1887	7	10	NULL	NULL	NULL	CREB	GP		bind					nNOS 	GP			CRE	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_15_8617_s_165	10900019	( D) CREB and ATF-2 bind to the nNOS CREs.	bind
2352	2	1887	7	10	NULL	NULL	NULL	ATF-2	GP		bind					 nNOS	GP			CRE	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_15_8617_s_165	10900019	( D) CREB and ATF-2 bind to the nNOS CREs.	bind
3017	1	1888	5	10	NULL	NULL	NULL	Sp1	GP		bind					p21WAF1/CIP1	GP			promoter	NULL	in high Ca2+-treated NHK cells	NULL	NULL	NULL	NULL	gw70_pnas_102_39_13921_s_149	16172401	( d) Cyclosporin A (CsA) abrogated the binding of Sp1 and NFAT1 to the p21WAF1/CIP1 promoter in high Ca2+-treated NHK cells, restoring the binding of KLF16, as assayed by a chromatin immunoprecipitation  assay.	bind
3018	2	1888	5	10	NULL	NULL	NULL	NFAT1	GP		bind					p21WAF1/CIP1	GP			promoter	NULL	in high Ca2+-treated NHK cells	NULL	NULL	NULL	NULL	gw70_pnas_102_39_13921_s_149	16172401	( d) Cyclosporin A (CsA) abrogated the binding of Sp1 and NFAT1 to the p21WAF1/CIP1 promoter in high Ca2+-treated NHK cells, restoring the binding of KLF16, as assayed by a chromatin immunoprecipitation  assay.	bind
3019	3	1888	5	10	NULL	NULL	NULL	CsA	Chemical		abrogate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_39_13921_s_149	16172401	( d) Cyclosporin A (CsA) abrogated the binding of Sp1 and NFAT1 to the p21WAF1/CIP1 promoter in high Ca2+-treated NHK cells, restoring the binding of KLF16, as assayed by a chromatin immunoprecipitation  assay.	bind
3020	4	1888	5	10	NULL	NULL	NULL	CsA	Chemical		is					Cyclosporin A	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_39_13921_s_149	16172401	( d) Cyclosporin A (CsA) abrogated the binding of Sp1 and NFAT1 to the p21WAF1/CIP1 promoter in high Ca2+-treated NHK cells, restoring the binding of KLF16, as assayed by a chromatin immunoprecipitation  assay.	bind
3021	5	1888	5	10	NULL	NULL	NULL	CsA	Chemical		abrogate					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_39_13921_s_149	16172401	( d) Cyclosporin A (CsA) abrogated the binding of Sp1 and NFAT1 to the p21WAF1/CIP1 promoter in high Ca2+-treated NHK cells, restoring the binding of KLF16, as assayed by a chromatin immunoprecipitation  assay.	bind
3022	6	1888	5	10	NULL	NULL	NULL	statement 3	Process		restore					KLF16	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_39_13921_s_149	16172401	( d) Cyclosporin A (CsA) abrogated the binding of Sp1 and NFAT1 to the p21WAF1/CIP1 promoter in high Ca2+-treated NHK cells, restoring the binding of KLF16, as assayed by a chromatin immunoprecipitation  assay.	bind
3023	7	1888	5	10	NULL	NULL	NULL	statement 5	Process		restore					KLF16	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_39_13921_s_149	16172401	( d) Cyclosporin A (CsA) abrogated the binding of Sp1 and NFAT1 to the p21WAF1/CIP1 promoter in high Ca2+-treated NHK cells, restoring the binding of KLF16, as assayed by a chromatin immunoprecipitation  assay.	bind
2353	1	1888	7	10	NULL	NULL	NULL	Sp1	GP		bind					p21WAF1/CIP1	GP			promoter	NULL	in high Ca2+-treated NHK cells	NULL	NULL	NULL	NULL	gw70_pnas_102_39_13921_s_149	16172401	( d) Cyclosporin A (CsA) abrogated the binding of Sp1 and NFAT1 to the p21WAF1/CIP1 promoter in high Ca2+-treated NHK cells, restoring the binding of KLF16, as assayed by a chromatin immunoprecipitation  assay.	bind
2354	2	1888	7	10	NULL	NULL	NULL	NFAT1	GP		bind					p21WAF1/CIP1	GP			promoter	NULL	in high Ca2+-treated NHK cells	NULL	NULL	NULL	NULL	gw70_pnas_102_39_13921_s_149	16172401	( d) Cyclosporin A (CsA) abrogated the binding of Sp1 and NFAT1 to the p21WAF1/CIP1 promoter in high Ca2+-treated NHK cells, restoring the binding of KLF16, as assayed by a chromatin immunoprecipitation  assay.	bind
2356	3	1888	7	10	NULL	NULL	NULL	CsA	Chemical		abrogates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_39_13921_s_149	16172401	( d) Cyclosporin A (CsA) abrogated the binding of Sp1 and NFAT1 to the p21WAF1/CIP1 promoter in high Ca2+-treated NHK cells, restoring the binding of KLF16, as assayed by a chromatin immunoprecipitation  assay.	bind
2357	4	1888	7	10	NULL	NULL	NULL	CsA	Chemical		abrogates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_39_13921_s_149	16172401	( d) Cyclosporin A (CsA) abrogated the binding of Sp1 and NFAT1 to the p21WAF1/CIP1 promoter in high Ca2+-treated NHK cells, restoring the binding of KLF16, as assayed by a chromatin immunoprecipitation  assay.	bind
51217	5	1888	7	10	NULL	NULL	NULL	CsA	Chemical		is					Cyclosporin A	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_39_13921_s_149	16172401	( d) Cyclosporin A (CsA) abrogated the binding of Sp1 and NFAT1 to the p21WAF1/CIP1 promoter in high Ca2+-treated NHK cells, restoring the binding of KLF16, as assayed by a chromatin immunoprecipitation  assay.	bind
51218	6	1888	7	10	NULL	NULL	NULL	statement 3	Process		restore					KLF16	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_39_13921_s_149	16172401	( d) Cyclosporin A (CsA) abrogated the binding of Sp1 and NFAT1 to the p21WAF1/CIP1 promoter in high Ca2+-treated NHK cells, restoring the binding of KLF16, as assayed by a chromatin immunoprecipitation  assay.	bind
51219	7	1888	7	10	NULL	NULL	NULL	statement 4	Process		restore					KLF16	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_39_13921_s_149	16172401	( d) Cyclosporin A (CsA) abrogated the binding of Sp1 and NFAT1 to the p21WAF1/CIP1 promoter in high Ca2+-treated NHK cells, restoring the binding of KLF16, as assayed by a chromatin immunoprecipitation  assay.	bind
3076	1	1889	5	10	NULL	NULL	NULL	HuR	GP	cellular	bind					IGF-IR	GP			5''-UTR	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_9_2962_s_167	15914670	( D) Demonstration of binding of cellular HuR to the IGF-IR 5''-UTR by altered mobility  on immunoblot (western-shift assay).	bind
2402	1	1889	7	10	NULL	NULL	NULL	HuR	GP	cellular	bind					IGF-IR	GP			5''-UTR	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_9_2962_s_167	15914670	( D) Demonstration of binding of cellular HuR to the IGF-IR 5''-UTR by altered mobility  on immunoblot (western-shift assay).	bind
3040	1	1890	5	10	NULL	NULL	NULL	pol	GP		bind		directly			PCNA	GP	monoubiquitinated			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_19_3886_s_225	15359278	( D) Direct binding of pol  to monoubiquitinated PCNA.	bind
2403	1	1890	7	10	NULL	NULL	NULL	pol	GP		binds to		directly			PCNA	GP	monoubiquitinated 			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_19_3886_s_225	15359278	( D) Direct binding of pol  to monoubiquitinated PCNA.	bind
3041	1	1891	5	10	NULL	NULL	NULL	PTEN	GP		bind		directly			NHERFs	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_910_s_60	16456542	( D) Direct binding of PTEN and PDGFR to NHERFs.	bind
3042	2	1891	5	10	NULL	NULL	NULL	PDGFR	GP		bind		directly			NHERFs	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_910_s_60	16456542	( D) Direct binding of PTEN and PDGFR to NHERFs.	bind
2404	1	1891	7	10	NULL	NULL	NULL	PTEN	GP		bind		directly			NHERFs	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_910_s_60	16456542	( D) Direct binding of PTEN and PDGFR to NHERFs.	bind
2405	2	1891	7	10	NULL	NULL	NULL	PDGFR	GP		bind		directly			NHERFs	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_910_s_60	16456542	( D) Direct binding of PTEN and PDGFR to NHERFs.	bind
3043	1	1892	5	10	NULL	NULL	NULL	GST-c-Src	GP	purified	bind		directly	SH3		integrin beta proteins	GP		cytoplasmic tail		NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_23_13298_s_112	14593208	( D) Direct binding of purified GST-c-Src SH3 to integrin beta cytoplasmic tail proteins, assessed by ELISA: beta3 ( ), rbeta3 ( ), beta3(delta758) ( ), beta1A ( ), and beta2 ( ).	bind
2406	1	1892	7	10	NULL	NULL	NULL	GST-c-Src	GP	purified	bind		directly	SH3		integrin beta proteins	GP		cytoplasmic tail 		NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_23_13298_s_112	14593208	( D) Direct binding of purified GST-c-Src SH3 to integrin beta cytoplasmic tail proteins, assessed by ELISA: beta3 ( ), rbeta3 ( ), beta3(delta758) ( ), beta1A ( ), and beta2 ( ).	bind
3044	1	1894	5	10	NULL	NULL	NULL	RNAP	GP		bind					A37	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_15_4245_s_126	16920742	( D) DNase I protection assay using RNAP bound to the  A37 promoter.	bind
2411	1	1894	7	10	NULL	NULL	NULL	RNAP	GP		bind					 A37	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_15_4245_s_126	16920742	( D) DNase I protection assay using RNAP bound to the  A37 promoter.	bind
3045	1	1895	5	10	NULL	NULL	NULL	Dsk2p	GP		bind					polyubiquitin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_2_745_s_110	11805328	( D) Dsk2p binds to polyubiquitin.	bind
2412	1	1895	7	10	NULL	NULL	NULL	Dsk2p	GP		bind					polyubiquitin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_2_745_s_110	11805328	( D) Dsk2p binds to polyubiquitin.	bind
3046	1	1896	5	10	NULL	NULL	NULL	E2F3	GP		bind					Cdc6	GP			promoter	NULL	at G1/S	NULL	NULL	NULL	NULL	gw60_embo_21_21_5775_s_161	12411495	( D) E2F3 but not E2F1 binds to the Cdc6 and RR1 promoter at G1/S.	bind
3047	2	1896	5	10	NULL	NULL	NULL	E2F3	GP		bind					RR1	GP			promoter	NULL	at G1/S	NULL	NULL	NULL	NULL	gw60_embo_21_21_5775_s_161	12411495	( D) E2F3 but not E2F1 binds to the Cdc6 and RR1 promoter at G1/S.	bind
3048	3	1896	5	10	NULL	NULL	NULL	E2F1	GP		does not bind					Cdc6	GP			promoter	NULL	at G1/S	NULL	NULL	NULL	NULL	gw60_embo_21_21_5775_s_161	12411495	( D) E2F3 but not E2F1 binds to the Cdc6 and RR1 promoter at G1/S.	bind
3049	4	1896	5	10	NULL	NULL	NULL	E2F1	GP		does not bind					RR1	GP			promoter	NULL	at G1/S	NULL	NULL	NULL	NULL	gw60_embo_21_21_5775_s_161	12411495	( D) E2F3 but not E2F1 binds to the Cdc6 and RR1 promoter at G1/S.	bind
2414	1	1896	7	10	NULL	NULL	NULL	E2F3	GP		bind					Cdc6	GP			promoter	NULL	at G1/S	NULL	NULL	NULL	NULL	gw60_embo_21_21_5775_s_161	12411495	( D) E2F3 but not E2F1 binds to the Cdc6 and RR1 promoter at G1/S.	bind
2415	2	1896	7	10	NULL	NULL	NULL	E2F3	GP		bind					RR1	GP			promoter	NULL	at G1/S	NULL	NULL	NULL	NULL	gw60_embo_21_21_5775_s_161	12411495	( D) E2F3 but not E2F1 binds to the Cdc6 and RR1 promoter at G1/S.	bind
2416	3	1896	7	10	NULL	NULL	NULL	E2F1	GP		does not bind					Cdc6	GP			promoter	NULL	at G1/S	NULL	NULL	NULL	NULL	gw60_embo_21_21_5775_s_161	12411495	( D) E2F3 but not E2F1 binds to the Cdc6 and RR1 promoter at G1/S.	bind
2417	4	1896	7	10	NULL	NULL	NULL	E2F1	GP		does not bind					RR1	GP			promoter	NULL	at G1/S	NULL	NULL	NULL	NULL	gw60_embo_21_21_5775_s_161	12411495	( D) E2F3 but not E2F1 binds to the Cdc6 and RR1 promoter at G1/S.	bind
3078	1	1897	5	10	NULL	NULL	NULL	EGF	GP		bind					EGFR/LckF505	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17896_s_167	8663450	( d) EGF binding to EGFR/LckF505 may allow the phosphorylation of the chimera by transphosphorylation of the EGFR/Lck dimer or phosphorylation by another PTK ( 60,  61) at Lck autophosphorylation site, Tyr-394, or possibly at the recently reported site within the Lck SH2 domain, Tyr-192 ( 62,  63).	bind
3079	2	1897	5	10	NULL	NULL	NULL	statement 1	Process		phosphorylate		may 			EGFR/LckF505	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17896_s_167	8663450	( d) EGF binding to EGFR/LckF505 may allow the phosphorylation of the chimera by transphosphorylation of the EGFR/Lck dimer or phosphorylation by another PTK ( 60,  61) at Lck autophosphorylation site, Tyr-394, or possibly at the recently reported site within the Lck SH2 domain, Tyr-192 ( 62,  63).	bind
3081	3	1897	5	10	NULL	NULL	NULL	statement 2	Process		occurs by					EGFR/Lck dimer	GP	transphosphorylation			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17896_s_167	8663450	( d) EGF binding to EGFR/LckF505 may allow the phosphorylation of the chimera by transphosphorylation of the EGFR/Lck dimer or phosphorylation by another PTK ( 60,  61) at Lck autophosphorylation site, Tyr-394, or possibly at the recently reported site within the Lck SH2 domain, Tyr-192 ( 62,  63).	bind
3082	4	1897	5	10	NULL	NULL	NULL	PTK	GP		phosphorylate					EGFR/Lck dimer	GP		Lck autophosphorylation site Tyr-394		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17896_s_167	8663450	( d) EGF binding to EGFR/LckF505 may allow the phosphorylation of the chimera by transphosphorylation of the EGFR/Lck dimer or phosphorylation by another PTK ( 60,  61) at Lck autophosphorylation site, Tyr-394, or possibly at the recently reported site within the Lck SH2 domain, Tyr-192 ( 62,  63).	bind
3083	5	1897	5	10	NULL	NULL	NULL	PTK	GP		phosphorylate					EGFR/Lck dimer	GP		Lck SH2 domain, Tyr-192		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17896_s_167	8663450	( d) EGF binding to EGFR/LckF505 may allow the phosphorylation of the chimera by transphosphorylation of the EGFR/Lck dimer or phosphorylation by another PTK ( 60,  61) at Lck autophosphorylation site, Tyr-394, or possibly at the recently reported site within the Lck SH2 domain, Tyr-192 ( 62,  63).	bind
3104	6	1897	5	10	NULL	NULL	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17896_s_167	8663450	( d) EGF binding to EGFR/LckF505 may allow the phosphorylation of the chimera by transphosphorylation of the EGFR/Lck dimer or phosphorylation by another PTK ( 60,  61) at Lck autophosphorylation site, Tyr-394, or possibly at the recently reported site within the Lck SH2 domain, Tyr-192 ( 62,  63).	bind
2419	1	1897	7	10	NULL	NULL	NULL	EGF	GP		bind					EGFR/LckF505 	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17896_s_167	8663450	( d) EGF binding to EGFR/LckF505 may allow the phosphorylation of the chimera by transphosphorylation of the EGFR/Lck dimer or phosphorylation by another PTK ( 60,  61) at Lck autophosphorylation site, Tyr-394, or possibly at the recently reported site within the Lck SH2 domain, Tyr-192 ( 62,  63).	bind
2420	2	1897	7	10	NULL	NULL	NULL	statement 1	Process		phosphorylate		may			EGFR/LckF505	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17896_s_167	8663450	( d) EGF binding to EGFR/LckF505 may allow the phosphorylation of the chimera by transphosphorylation of the EGFR/Lck dimer or phosphorylation by another PTK ( 60,  61) at Lck autophosphorylation site, Tyr-394, or possibly at the recently reported site within the Lck SH2 domain, Tyr-192 ( 62,  63).	bind
2421	3	1897	7	10	NULL	NULL	NULL	statement 2	Process		occurs through					EGFR/Lck dimer	GP	transphosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17896_s_167	8663450	( d) EGF binding to EGFR/LckF505 may allow the phosphorylation of the chimera by transphosphorylation of the EGFR/Lck dimer or phosphorylation by another PTK ( 60,  61) at Lck autophosphorylation site, Tyr-394, or possibly at the recently reported site within the Lck SH2 domain, Tyr-192 ( 62,  63).	bind
2422	4	1897	7	10	NULL	NULL	NULL	PTK	GP		phosphorylate					EGFR/LckF505	GP		Lck autophosphorylation site, Tyr-394		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17896_s_167	8663450	( d) EGF binding to EGFR/LckF505 may allow the phosphorylation of the chimera by transphosphorylation of the EGFR/Lck dimer or phosphorylation by another PTK ( 60,  61) at Lck autophosphorylation site, Tyr-394, or possibly at the recently reported site within the Lck SH2 domain, Tyr-192 ( 62,  63).	bind
2423	5	1897	7	10	NULL	NULL	NULL	PTK	GP		phosphorylate					EGFR/LckF505	GP		Lck SH2 domain, Tyr-192		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17896_s_167	8663450	( d) EGF binding to EGFR/LckF505 may allow the phosphorylation of the chimera by transphosphorylation of the EGFR/Lck dimer or phosphorylation by another PTK ( 60,  61) at Lck autophosphorylation site, Tyr-394, or possibly at the recently reported site within the Lck SH2 domain, Tyr-192 ( 62,  63).	bind
2424	6	1897	7	10	NULL	NULL	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17896_s_167	8663450	( d) EGF binding to EGFR/LckF505 may allow the phosphorylation of the chimera by transphosphorylation of the EGFR/Lck dimer or phosphorylation by another PTK ( 60,  61) at Lck autophosphorylation site, Tyr-394, or possibly at the recently reported site within the Lck SH2 domain, Tyr-192 ( 62,  63).	bind
3050	1	1898	5	10	NULL	NULL	NULL	EGL-17	GP		bind					Ce-LRP-2	GP		YWTD region		NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_22_2798_s_205	14630941	( D) EGL-17 binds to Ce-LRP-2 YWTD region.	bind
2418	1	1898	7	10	NULL	NULL	NULL	EGL-17	GP		bind					Ce-LRP-2	GP		YWTD		NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_22_2798_s_205	14630941	( D) EGL-17 binds to Ce-LRP-2 YWTD region.	bind
3051	1	1899	5	10	NULL	NULL	NULL	AEBP1	GP		bind		specifically			hPPARgamma1	GP			AE-1 homologous sequences in the promoter	NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_7_2346_s_64	16461908	( D) EMSA shows that AEBP1 specifically binds to AE-1 homologous sequences in the promoter  regions of hPPARgamma1 and mLXRalpha but not to the mutated sequences (hPPARgamma1-M and mLXRalpha-M).	bind
3052	2	1899	5	10	NULL	NULL	NULL	AEBP1	GP		bind		specifically			mLXRalpha	GP			AE-1 homologous sequences in the promoter	NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_7_2346_s_64	16461908	( D) EMSA shows that AEBP1 specifically binds to AE-1 homologous sequences in the promoter  regions of hPPARgamma1 and mLXRalpha but not to the mutated sequences (hPPARgamma1-M and mLXRalpha-M).	bind
3053	3	1899	5	10	NULL	NULL	NULL	AEBP1	GP		does not bind					hPPARgamma1-M	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_7_2346_s_64	16461908	( D) EMSA shows that AEBP1 specifically binds to AE-1 homologous sequences in the promoter  regions of hPPARgamma1 and mLXRalpha but not to the mutated sequences (hPPARgamma1-M and mLXRalpha-M).	bind
3054	4	1899	5	10	NULL	NULL	NULL	AEBP1	GP		does not bind					mLXRalpha-M	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_7_2346_s_64	16461908	( D) EMSA shows that AEBP1 specifically binds to AE-1 homologous sequences in the promoter  regions of hPPARgamma1 and mLXRalpha but not to the mutated sequences (hPPARgamma1-M and mLXRalpha-M).	bind
2425	1	1899	7	10	NULL	NULL	NULL	AEBP1	GP		binds to		specifically			hPPARgamma1	GP			 AE-1 homologous sequences in the promoter of 	NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_7_2346_s_64	16461908	( D) EMSA shows that AEBP1 specifically binds to AE-1 homologous sequences in the promoter  regions of hPPARgamma1 and mLXRalpha but not to the mutated sequences (hPPARgamma1-M and mLXRalpha-M).	bind
2426	2	1899	7	10	NULL	NULL	NULL	AEBP1	GP		binds to		specifically			mLXRalpha	GP			AE-1 homologous sequences in the promoter of	NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_7_2346_s_64	16461908	( D) EMSA shows that AEBP1 specifically binds to AE-1 homologous sequences in the promoter  regions of hPPARgamma1 and mLXRalpha but not to the mutated sequences (hPPARgamma1-M and mLXRalpha-M).	bind
2427	3	1899	7	10	NULL	NULL	NULL	AEBP1	GP		does not bind					hPPARgamma1-M	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_7_2346_s_64	16461908	( D) EMSA shows that AEBP1 specifically binds to AE-1 homologous sequences in the promoter  regions of hPPARgamma1 and mLXRalpha but not to the mutated sequences (hPPARgamma1-M and mLXRalpha-M).	bind
2428	4	1899	7	10	NULL	NULL	NULL	AEBP1	GP		does not bind					mLXRalpha-M	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_7_2346_s_64	16461908	( D) EMSA shows that AEBP1 specifically binds to AE-1 homologous sequences in the promoter  regions of hPPARgamma1 and mLXRalpha but not to the mutated sequences (hPPARgamma1-M and mLXRalpha-M).	bind
3055	1	1900	5	10	NULL	NULL	NULL	SLP-76	GP		bind					PLCgamma1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_12_1762_s_231	15599401	( D) EphB6 augmented binding of SLP-76 with PLCgamma1 after TCR activation.	bind
3056	2	1900	5	10	NULL	NULL	NULL	statement 1	Process		occurs following					TCR	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_12_1762_s_231	15599401	( D) EphB6 augmented binding of SLP-76 with PLCgamma1 after TCR activation.	bind
3057	3	1900	5	10	NULL	NULL	NULL	EphB6	GP		augment					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_12_1762_s_231	15599401	( D) EphB6 augmented binding of SLP-76 with PLCgamma1 after TCR activation.	bind
2431	1	1900	7	10	NULL	NULL	NULL	SLP-76	GP		bind					PLCgamma1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_12_1762_s_231	15599401	( D) EphB6 augmented binding of SLP-76 with PLCgamma1 after TCR activation.	bind
2432	2	1900	7	10	NULL	NULL	NULL	 EphB6	GP		augment					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_12_1762_s_231	15599401	( D) EphB6 augmented binding of SLP-76 with PLCgamma1 after TCR activation.	bind
2433	3	1900	7	10	NULL	NULL	NULL	statement 2	Process		occurs after					TCR	GP	activation of 			NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_12_1762_s_231	15599401	( D) EphB6 augmented binding of SLP-76 with PLCgamma1 after TCR activation.	bind
3058	1	1901	5	10	NULL	NULL	NULL	ERs	GP		does not bind					TNF	GP			RE	NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_26_15161_s_99	10611355	( D) ERs do not bind to the TNF-RE.	bind
3202	1	1901	7	10	NULL	NULL	NULL	ERs	GP		does not bind					TNF	GP			RE	NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_26_15161_s_99	10611355	( D) ERs do not bind to the TNF-RE.	bind
3059	1	1902	5	10	NULL	NULL	NULL	PB1	GP		bind					vRNA oligonucleotide	NucleicAcid	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_429_s_189	11788704	( D) Estimation of the quantity of PB1 bound to the immobilised vRNA oligonucleotide.	bind
3204	1	1902	7	10	NULL	NULL	NULL	PB1	GP		bind					vRNA oligonucleotide	NucleicAcid	immobilised			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_429_s_189	11788704	( D) Estimation of the quantity of PB1 bound to the immobilised vRNA oligonucleotide.	bind
3060	1	1904	5	10	NULL	NULL	NULL	Fbw7	GP		bind		preferentially			cyclin E-Cdk2	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_294_5540_173_s_53	11533444	( D) Fbw7 preferentially binds cyclin E-Cdk2.	bind
3206	1	1904	7	10	NULL	NULL	NULL	Fbw7	GP		bind		preferentially			cyclin E-Cdk2	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_294_5540_173_s_53	11533444	( D) Fbw7 preferentially binds cyclin E-Cdk2.	bind
3061	1	1905	5	10	NULL	NULL	NULL	Fhl1	GP		bind		specifically			 RP	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_18_20_2491_s_279	15466158	( D) Fhl1 and Ifh1 bind specifically to  RP promoters.	bind
3062	2	1905	5	10	NULL	NULL	NULL	Ifh1	GP		bind		specifically			RP	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_18_20_2491_s_279	15466158	( D) Fhl1 and Ifh1 bind specifically to  RP promoters.	bind
3207	1	1905	7	10	NULL	NULL	NULL	Fhl1	GP		bind		specifically			RP	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_18_20_2491_s_279	15466158	( D) Fhl1 and Ifh1 bind specifically to  RP promoters.	bind
3208	2	1905	7	10	NULL	NULL	NULL	 Ifh1	GP		bind		specifically			RP	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_18_20_2491_s_279	15466158	( D) Fhl1 and Ifh1 bind specifically to  RP promoters.	bind
3063	1	1906	5	10	NULL	NULL	NULL	mAb 1D11	GP		bind					Jurkat-NKG2D	Cell	transfectants			NULL		NULL	NULL	NULL	NULL	gw60_science_285_5428_727_s_71	10426993	( D) Flow cytometry showed binding of mAb 1D11 to the Jurkat-NKG2D transfectants but not to the untransfected cells.	bind
3064	2	1906	5	10	NULL	NULL	NULL	mAb 1D11	GP		does not bind					untransfected cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_science_285_5428_727_s_71	10426993	( D) Flow cytometry showed binding of mAb 1D11 to the Jurkat-NKG2D transfectants but not to the untransfected cells.	bind
3217	1	1906	7	10	NULL	NULL	NULL	mAb 1D11	GP		bind					 Jurkat-NKG2D 	Cell	transfectants			NULL		NULL	NULL	NULL	NULL	gw60_science_285_5428_727_s_71	10426993	( D) Flow cytometry showed binding of mAb 1D11 to the Jurkat-NKG2D transfectants but not to the untransfected cells.	bind
3218	2	1906	7	10	NULL	NULL	NULL	mAb 1D11	GP		does not bind					untransfected cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_science_285_5428_727_s_71	10426993	( D) Flow cytometry showed binding of mAb 1D11 to the Jurkat-NKG2D transfectants but not to the untransfected cells.	bind
3065	1	1907	5	10	NULL	NULL	NULL	GA	GP		bind					TfR	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_34_12095_s_105	16103367	( D) GA binds to TfR.	bind
3219	1	1907	7	10	NULL	NULL	NULL	GA	GP		bind					 TfR	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_34_12095_s_105	16103367	( D) GA binds to TfR.	bind
3066	1	1909	5	10	NULL	NULL	NULL	GST-Aly	GP		bind					ORF57	GP	WT			NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_41_15190_s_124	17005724	( d) GST pull-down assays were repeated to compare the binding affinity of GST-Aly with  WT ORF57 and ORF57NLS1M.	bind
3067	2	1909	5	10	NULL	NULL	NULL	GST-Aly	GP		bind					ORF57	GP		NLS1M		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_41_15190_s_124	17005724	( d) GST pull-down assays were repeated to compare the binding affinity of GST-Aly with  WT ORF57 and ORF57NLS1M.	bind
3220	1	1909	7	10	NULL	NULL	NULL	GST-Aly	GP		bind					 ORF57	GP	WT 			NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_41_15190_s_124	17005724	( d) GST pull-down assays were repeated to compare the binding affinity of GST-Aly with  WT ORF57 and ORF57NLS1M.	bind
3221	2	1909	7	10	NULL	NULL	NULL	GST-Aly	GP		bind					ORF57	GP		NLS1M		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_41_15190_s_124	17005724	( d) GST pull-down assays were repeated to compare the binding affinity of GST-Aly with  WT ORF57 and ORF57NLS1M.	bind
3068	1	1910	5	10	NULL	NULL	NULL	HBP1	GP		does not bind									LEF/TCF DNA binding site	NULL		NULL	NULL	NULL	NULL	gw60_embo_20_16_4500_s_160	11500377	( D) HBP1 does not bind the TOPFLASH LEF/TCF DNA binding site.	bind
3222	1	1910	7	10	NULL	NULL	NULL	HBP1	GP		does not bind									 LEF/TCF DNA binding site	NULL		NULL	NULL	NULL	NULL	gw60_embo_20_16_4500_s_160	11500377	( D) HBP1 does not bind the TOPFLASH LEF/TCF DNA binding site.	bind
3327	1	1911	5	10	NULL	NULL	NULL	FGF-2	GP		bind					Namalwa-CD44vRA	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_111_8_1211_s_135	12697740	( d) Heparinase treatment reduces FGF-2 binding to Namalwa-CD44vRA.	bind
3328	2	1911	5	10	NULL	NULL	NULL	Heparinase	GP		reduce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_111_8_1211_s_135	12697740	( d) Heparinase treatment reduces FGF-2 binding to Namalwa-CD44vRA.	bind
3223	1	1911	7	10	NULL	NULL	NULL	FGF-2	GP		bind					Namalwa CD44vRA	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_111_8_1211_s_135	12697740	( d) Heparinase treatment reduces FGF-2 binding to Namalwa-CD44vRA.	bind
3224	2	1911	7	10	NULL	NULL	NULL	Heparinase	GP		reduces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_111_8_1211_s_135	12697740	( d) Heparinase treatment reduces FGF-2 binding to Namalwa-CD44vRA.	bind
3329	1	1912	5	10	NULL	NULL	NULL	HsdR	GP		bind					MTase	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_23_4188_s_102	16292342	( D) HsdR binding rate to the MTase at different HsdR concentrations obtained from fitting  the triplex displacement curves.	bind
3225	1	1912	7	10	NULL	NULL	NULL	HsdR	GP		binds to					MTase	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_23_4188_s_102	16292342	( D) HsdR binding rate to the MTase at different HsdR concentrations obtained from fitting  the triplex displacement curves.	bind
3331	1	1913	5	10	NULL	NULL	NULL	hTAFII130	GP		bind					HP1alpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_9_5919_s_128	11959914	( D) hTAFII130 bound to HP1alpha and HP1gamma but not to HP1beta.	bind
3332	2	1913	5	10	NULL	NULL	NULL	hTAFII130	GP		bind					HP1gamma	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_9_5919_s_128	11959914	( D) hTAFII130 bound to HP1alpha and HP1gamma but not to HP1beta.	bind
3333	3	1913	5	10	NULL	NULL	NULL	hTAFII130	GP		does not bind					HP1beta	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_9_5919_s_128	11959914	( D) hTAFII130 bound to HP1alpha and HP1gamma but not to HP1beta.	bind
3226	1	1913	7	10	NULL	NULL	NULL	hTAFII130	GP		bind					HP1alpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_9_5919_s_128	11959914	( D) hTAFII130 bound to HP1alpha and HP1gamma but not to HP1beta.	bind
3227	2	1913	7	10	NULL	NULL	NULL	hTAFII130	GP		bind					HP1gamma 	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_9_5919_s_128	11959914	( D) hTAFII130 bound to HP1alpha and HP1gamma but not to HP1beta.	bind
3228	3	1913	7	10	NULL	NULL	NULL	 hTAFII130	GP		does not bind					HP1beta	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_9_5919_s_128	11959914	( D) hTAFII130 bound to HP1alpha and HP1gamma but not to HP1beta.	bind
3334	1	1915	5	10	NULL	NULL	NULL	ICSBP	GP		bind					Dab2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_21_3_211_s_65	11823414	( D) ICSBP and PU.1 bind to the Dab2 promoter.	bind
3335	2	1915	5	10	NULL	NULL	NULL	PU.1	GP		bind					Dab2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_21_3_211_s_65	11823414	( D) ICSBP and PU.1 bind to the Dab2 promoter.	bind
3230	1	1915	7	10	NULL	NULL	NULL	ICSBP	GP		bind					Dab2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_21_3_211_s_65	11823414	( D) ICSBP and PU.1 bind to the Dab2 promoter.	bind
3231	2	1915	7	10	NULL	NULL	NULL	PU.1	GP		bind					Dab2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_21_3_211_s_65	11823414	( D) ICSBP and PU.1 bind to the Dab2 promoter.	bind
3336	1	1916	5	10	NULL	NULL	NULL	poliota	GP		bind					Ub	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_12_2847_s_49	16763556	( D) In addition to poliota, pol  also binds to Ub.	bind
3337	2	1916	5	10	NULL	NULL	NULL	pol	GP		bind					Ub	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_12_2847_s_49	16763556	( D) In addition to poliota, pol  also binds to Ub.	bind
3232	1	1916	7	10	NULL	NULL	NULL	poliota	GP		bind					Ub	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_12_2847_s_49	16763556	( D) In addition to poliota, pol  also binds to Ub.	bind
3233	2	1916	7	10	NULL	NULL	NULL	pol	GP		bind					Ub	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_12_2847_s_49	16763556	( D) In addition to poliota, pol  also binds to Ub.	bind
3442	1	1917	5	10	NULL	NULL	NULL	annexin-V biotin	GP		bind					K5/rTA DT	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_16_9139_s_139	11481479	( D) Increased annexin-V biotin binding of K5/rTA DT but not control keratinocytes 48 h after addition of doxycycline.	bind
3443	2	1917	5	10	NULL	NULL	NULL	doxycycline	Chemical	addition	increase					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_16_9139_s_139	11481479	( D) Increased annexin-V biotin binding of K5/rTA DT but not control keratinocytes 48 h after addition of doxycycline.	bind
3444	3	1917	5	10	NULL	NULL	NULL	annexin-V biotin	GP		does not bind					keratinocytes	Cell	control			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_16_9139_s_139	11481479	( D) Increased annexin-V biotin binding of K5/rTA DT but not control keratinocytes 48 h after addition of doxycycline.	bind
3235	1	1917	7	10	NULL	NULL	NULL	annexin-V biotin	GP		bind					K5/rTA DT	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_16_9139_s_139	11481479	( D) Increased annexin-V biotin binding of K5/rTA DT but not control keratinocytes 48 h after addition of doxycycline.	bind
3237	2	1917	7	10	NULL	NULL	NULL	annexin-V biotin	GP		does not bind					 keratinocytes	Cell				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_16_9139_s_139	11481479	( D) Increased annexin-V biotin binding of K5/rTA DT but not control keratinocytes 48 h after addition of doxycycline.	bind
4596	3	1917	7	10	NULL	NULL	NULL	doxycycline	Chemical	addition	increase					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_16_9139_s_139	11481479	( D) Increased annexin-V biotin binding of K5/rTA DT but not control keratinocytes 48 h after addition of doxycycline.	bind
3490	1	1918	5	10	NULL	NULL	NULL	calmodulin	GP	rat brain;; cytosolic	bind					mGluR 7	GP		tail regions		NULL		NULL	NULL	NULL	NULL	gw60_science_286_5442_1180_s_38	10550060	( D) Incubating rat brain cytosolic proteins with GST, GST-7A, or GST-7B in the presence of CaCl2 (1 mM) or EGTA (5 mM) revealed that the binding of calmodulin to the mGluR 7 tail regions is Ca2+- dependent.	bind
3491	2	1918	5	10	NULL	NULL	NULL	statement 1	Process		is dependent on					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5442_1180_s_38	10550060	( D) Incubating rat brain cytosolic proteins with GST, GST-7A, or GST-7B in the presence of CaCl2 (1 mM) or EGTA (5 mM) revealed that the binding of calmodulin to the mGluR 7 tail regions is Ca2+- dependent.	bind
3240	1	1918	7	10	NULL	NULL	NULL	calmodulin	GP	rat brain;; cytosolic	bind					mGluR 7	GP		tail region		NULL		NULL	NULL	NULL	NULL	gw60_science_286_5442_1180_s_38	10550060	( D) Incubating rat brain cytosolic proteins with GST, GST-7A, or GST-7B in the presence of CaCl2 (1 mM) or EGTA (5 mM) revealed that the binding of calmodulin to the mGluR 7 tail regions is Ca2+- dependent.	bind
3241	2	1918	7	10	NULL	NULL	NULL	statement 1	Process		is dependent on					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5442_1180_s_38	10550060	( D) Incubating rat brain cytosolic proteins with GST, GST-7A, or GST-7B in the presence of CaCl2 (1 mM) or EGTA (5 mM) revealed that the binding of calmodulin to the mGluR 7 tail regions is Ca2+- dependent.	bind
3495	2	1919	5	10	NULL	NULL	NULL	rGL-7	GP		induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_13_7454_s_142	12802014	( D) Induction of  NAD+ glycohydrolase activity by rGL-7.	bind
46204	1	1919	5	10	NULL	NULL	NULL	NAD+	Chemical		activates					glycohydrolase 	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_13_7454_s_142	12802014	( D) Induction of  NAD+ glycohydrolase activity by rGL-7.	bind
46208	1	1919	7	10	NULL	NULL	NULL	NAD+	Chemical		activates					glycohydrolase 	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_13_7454_s_142	12802014	( D) Induction of  NAD+ glycohydrolase activity by rGL-7.	bind
46209	2	1919	7	10	NULL	NULL	NULL	 rGL-7	GP		induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_13_7454_s_142	12802014	( D) Induction of  NAD+ glycohydrolase activity by rGL-7.	bind
3496	1	1920	5	10	NULL	NULL	NULL	IpaA	GP		does not bind					F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_5853_s_185	10545097	( D) IpaA does not bind to F-actin.	bind
3243	1	1920	7	10	NULL	NULL	NULL	IpaA	GP		does not bind					F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_5853_s_185	10545097	( D) IpaA does not bind to F-actin.	bind
3497	1	1921	5	10	NULL	NULL	NULL	ubiquitin	GP		bind					HDAC6	GP		ZnF-UBP		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_14_3357_s_40	16810319	( D) ITC profile for the binding of ubiquitin to HDAC6 ZnF-UBP.	bind
3244	1	1921	7	10	NULL	NULL	NULL	ubiquitin	GP		bind					HDAC6	GP		 ZnF-UBP		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_14_3357_s_40	16810319	( D) ITC profile for the binding of ubiquitin to HDAC6 ZnF-UBP.	bind
3498	1	1922	5	10	NULL	NULL	NULL	JunB	GP		does not bind					PPARbeta	GP			AP-1 site of promoter	NULL		NULL	NULL	NULL	NULL	gw70_embo_23_21_4211_s_107	15470497	( D) JunB is not binding to the AP-1 site of the PPARbeta promoter.	bind
3245	1	1922	7	10	NULL	NULL	NULL	JunB	GP		does not bind					PPARbeta	GP			AP-1 site promoter of	NULL		NULL	NULL	NULL	NULL	gw70_embo_23_21_4211_s_107	15470497	( D) JunB is not binding to the AP-1 site of the PPARbeta promoter.	bind
3795	1	1923	5	10	NULL	NULL	NULL	L-Sox5	GP		bind									48 bp probe	NULL		NULL	NULL	NULL	NULL	gw60_embo_17_19_5718_s_91	9755172	( D) L-Sox5, Sox6 and SOX9 bound to the 48 bp probe.	bind
3796	2	1923	5	10	NULL	NULL	NULL	Sox6	GP		bind									48 bp probe	NULL		NULL	NULL	NULL	NULL	gw60_embo_17_19_5718_s_91	9755172	( D) L-Sox5, Sox6 and SOX9 bound to the 48 bp probe.	bind
3797	3	1923	5	10	NULL	NULL	NULL	SOX9	GP		bind									48 bp probe	NULL		NULL	NULL	NULL	NULL	gw60_embo_17_19_5718_s_91	9755172	( D) L-Sox5, Sox6 and SOX9 bound to the 48 bp probe.	bind
3246	1	1923	7	10	NULL	NULL	NULL	L-Sox5	GP		 bind									48 bp probe	NULL		NULL	NULL	NULL	NULL	gw60_embo_17_19_5718_s_91	9755172	( D) L-Sox5, Sox6 and SOX9 bound to the 48 bp probe.	bind
3247	2	1923	7	10	NULL	NULL	NULL	Sox6	GP		bind									48 bp probe	NULL		NULL	NULL	NULL	NULL	gw60_embo_17_19_5718_s_91	9755172	( D) L-Sox5, Sox6 and SOX9 bound to the 48 bp probe.	bind
3248	3	1923	7	10	NULL	NULL	NULL	SOX9 	GP		bind									48 bp probe	NULL		NULL	NULL	NULL	NULL	gw60_embo_17_19_5718_s_91	9755172	( D) L-Sox5, Sox6 and SOX9 bound to the 48 bp probe.	bind
3501	1	1924	5	10	NULL	NULL	NULL	STAT3	GP		bind					Nanog	GP	putative		STAT-binding site in regulatory region	NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_27_10294_s_46	16801560	( D) LIF-dependent binding of STAT3 to the putative STAT-binding site in the  Nanog regulatory region.	bind
3502	2	1924	5	10	NULL	NULL	NULL	statement 1	Process		is dependent on					LIF	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_27_10294_s_46	16801560	( D) LIF-dependent binding of STAT3 to the putative STAT-binding site in the  Nanog regulatory region.	bind
3249	1	1924	7	10	NULL	NULL	NULL	STAT3	GP		bind					Nanog	GP	putative		STAT-binding site regulatory region	NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_27_10294_s_46	16801560	( D) LIF-dependent binding of STAT3 to the putative STAT-binding site in the  Nanog regulatory region.	bind
3250	2	1924	7	10	NULL	NULL	NULL	statement 1	Process		is dependent  on					LIF	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_27_10294_s_46	16801560	( D) LIF-dependent binding of STAT3 to the putative STAT-binding site in the  Nanog regulatory region.	bind
3504	1	1925	5	10	NULL	NULL	NULL	SB203580	Chemical		is a type of					MAP kinase inhibitor	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_10_1162_s_211	15870257	( D) MAP kinase inhibitor SB203580 completely abrogates p38 MAP kinase activity.	bind
3505	2	1925	5	10	NULL	NULL	NULL	SB203580	Chemical		abrogate		completely			p38 MAP kinase	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_10_1162_s_211	15870257	( D) MAP kinase inhibitor SB203580 completely abrogates p38 MAP kinase activity.	bind
3267	1	1925	7	10	NULL	NULL	NULL	SB203580	Chemical		abrogates		completely			p38 MAP kinase 	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_10_1162_s_211	15870257	( D) MAP kinase inhibitor SB203580 completely abrogates p38 MAP kinase activity.	bind
4597	2	1925	7	10	NULL	NULL	NULL	SB203580 	Chemical		is a type of					MAP kinase inhibitor	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_10_1162_s_211	15870257	( D) MAP kinase inhibitor SB203580 completely abrogates p38 MAP kinase activity.	bind
3508	1	1927	5	10	NULL	NULL	NULL	MBP - Kap114p	GP		bind					GST - histone	GP		N-terminal tail		NULL		NULL	NULL	NULL	NULL	gw60_embo_21_23_6527_s_106	12456659	( D) MBP - Kap114p (200 nM) binding to GST - histone N-terminal tails as in (B).	bind
3268	1	1927	7	10	NULL	NULL	NULL	MBP - Kap114p	GP		bind					GST - histone	GP		N-terminal tails		NULL		NULL	NULL	NULL	NULL	gw60_embo_21_23_6527_s_106	12456659	( D) MBP - Kap114p (200 nM) binding to GST - histone N-terminal tails as in (B).	bind
3509	1	1930	5	10	NULL	NULL	NULL	TF1-v1	GP		bind					theophylline	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_7_1631_s_153	11266567	( D) Model of TF1-v1 bound to theophylline and FMN (encircled F).	bind
3510	2	1930	5	10	NULL	NULL	NULL	TF1-v1	GP		bind					FMN	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_7_1631_s_153	11266567	( D) Model of TF1-v1 bound to theophylline and FMN (encircled F).	bind
3269	1	1930	7	10	NULL	NULL	NULL	TF1-v1	GP		bind					theophylline	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_7_1631_s_153	11266567	( D) Model of TF1-v1 bound to theophylline and FMN (encircled F).	bind
3270	2	1930	7	10	NULL	NULL	NULL	TF1-v1	GP		bind					FMN	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_7_1631_s_153	11266567	( D) Model of TF1-v1 bound to theophylline and FMN (encircled F).	bind
3512	1	1931	5	10	NULL	NULL	NULL	MTA-1	GP		bind					GST-FOG-1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_embo_24_13_2367_s_140	15920470	( D) MTA-1, MTA-2 and RbAP48 bind GST-FOG-1(45)  in vitro.	bind
3513	2	1931	5	10	NULL	NULL	NULL	MTA-2	GP		bind					GST-FOG-1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_embo_24_13_2367_s_140	15920470	( D) MTA-1, MTA-2 and RbAP48 bind GST-FOG-1(45)  in vitro.	bind
3514	3	1931	5	10	NULL	NULL	NULL	RbAP48	GP		bind					GST-FOG-1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_embo_24_13_2367_s_140	15920470	( D) MTA-1, MTA-2 and RbAP48 bind GST-FOG-1(45)  in vitro.	bind
3271	1	1931	7	10	NULL	NULL	NULL	MTA-1	GP		bind					GST-FOG-1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_embo_24_13_2367_s_140	15920470	( D) MTA-1, MTA-2 and RbAP48 bind GST-FOG-1(45)  in vitro.	bind
3272	2	1931	7	10	NULL	NULL	NULL	MTA-2	GP		bind					GST-FOG-1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_embo_24_13_2367_s_140	15920470	( D) MTA-1, MTA-2 and RbAP48 bind GST-FOG-1(45)  in vitro.	bind
3273	3	1931	7	10	NULL	NULL	NULL	RbAP48	GP		bind					GST-FOG-1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_embo_24_13_2367_s_140	15920470	( D) MTA-1, MTA-2 and RbAP48 bind GST-FOG-1(45)  in vitro.	bind
3515	1	1932	5	10	NULL	NULL	NULL	GST-N-CFTR	GP		bind					syn1AdeltaC	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_18_10972_s_86	9724814	( D) Munc-18a blocks the binding of GST-N-CFTR to syn1AdeltaC.	bind
3516	2	1932	5	10	NULL	NULL	NULL	Munc-18a	GP		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_18_10972_s_86	9724814	( D) Munc-18a blocks the binding of GST-N-CFTR to syn1AdeltaC.	bind
3274	1	1932	7	10	NULL	NULL	NULL	GST-N-CFTR	GP		bind					syn1AdeltaC	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_18_10972_s_86	9724814	( D) Munc-18a blocks the binding of GST-N-CFTR to syn1AdeltaC.	bind
3275	2	1932	7	10	NULL	NULL	NULL	Munc-18a	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_18_10972_s_86	9724814	( D) Munc-18a blocks the binding of GST-N-CFTR to syn1AdeltaC.	bind
3523	1	1933	5	10	NULL	NULL	NULL	importin-alpha	GP		is					Kap60p	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_21_3681_s_121	16222336	( D) Mutants in the Nup2p residues analogous to those identified in the two importin-alpha-binding regions of Nup50 do not displace the monopartite or bipartite NLSs from yeast  importin-alpha (Kap60p).	bind
3528	2	1933	5	10	NULL	NULL	NULL	Nup2p	GP	mutant	analogus to					Nup50	GP		 importin-alpha-binding regions		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_21_3681_s_121	16222336	( D) Mutants in the Nup2p residues analogous to those identified in the two importin-alpha-binding regions of Nup50 do not displace the monopartite or bipartite NLSs from yeast  importin-alpha (Kap60p).	bind
3530	3	1933	5	10	NULL	NULL	NULL	statement 2	Process		does not displace					 importin-alpha	GP	yeast	monopartite NLS		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_21_3681_s_121	16222336	( D) Mutants in the Nup2p residues analogous to those identified in the two importin-alpha-binding regions of Nup50 do not displace the monopartite or bipartite NLSs from yeast  importin-alpha (Kap60p).	bind
3531	4	1933	5	10	NULL	NULL	NULL	statement 2	Process		does not displace					importin-alpha	GP	yeast	bipartite NLS		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_21_3681_s_121	16222336	( D) Mutants in the Nup2p residues analogous to those identified in the two importin-alpha-binding regions of Nup50 do not displace the monopartite or bipartite NLSs from yeast  importin-alpha (Kap60p).	bind
3276	1	1933	7	10	NULL	NULL	NULL	Nup2p	GP	mutant	does not displace					importin-alpha	GP	yeast	monopartite NLSs		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_21_3681_s_121	16222336	( D) Mutants in the Nup2p residues analogous to those identified in the two importin-alpha-binding regions of Nup50 do not displace the monopartite or bipartite NLSs from yeast  importin-alpha (Kap60p).	bind
3277	2	1933	7	10	NULL	NULL	NULL	Nup2p	GP	mutant	does not displace					importin-alpha 	GP	yeast	bipartite NLSs		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_21_3681_s_121	16222336	( D) Mutants in the Nup2p residues analogous to those identified in the two importin-alpha-binding regions of Nup50 do not displace the monopartite or bipartite NLSs from yeast  importin-alpha (Kap60p).	bind
3278	3	1933	7	10	NULL	NULL	NULL	Nup2p 	GP	Mutant	is analogous 			residues		Nup50	GP		two importin-alpha-binding regions		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_21_3681_s_121	16222336	( D) Mutants in the Nup2p residues analogous to those identified in the two importin-alpha-binding regions of Nup50 do not displace the monopartite or bipartite NLSs from yeast  importin-alpha (Kap60p).	bind
3279	4	1933	7	10	NULL	NULL	NULL	importin-alpha	GP		is					Kap60p	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_21_3681_s_121	16222336	( D) Mutants in the Nup2p residues analogous to those identified in the two importin-alpha-binding regions of Nup50 do not displace the monopartite or bipartite NLSs from yeast  importin-alpha (Kap60p).	bind
3520	1	1934	5	10	NULL	NULL	NULL	Myc	GP		bind		directly			Dnmt3a	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_2_336_s_161	15616584	( D) Myc binds directly to Dnmt3a, whereas Miz-1 only weakly binds directly to Dnmt3a.	bind
3522	2	1934	5	10	NULL	NULL	NULL	Miz-1	GP		bind		weakly			Dnmt3a	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_2_336_s_161	15616584	( D) Myc binds directly to Dnmt3a, whereas Miz-1 only weakly binds directly to Dnmt3a.	bind
3280	1	1934	7	10	NULL	NULL	NULL	Myc	GP		binds		directly			Dnmt3a	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_2_336_s_161	15616584	( D) Myc binds directly to Dnmt3a, whereas Miz-1 only weakly binds directly to Dnmt3a.	bind
3281	2	1934	7	10	NULL	NULL	NULL	Miz-1	GP		binds		weakly			Dnmt3a	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_2_336_s_161	15616584	( D) Myc binds directly to Dnmt3a, whereas Miz-1 only weakly binds directly to Dnmt3a.	bind
3518	1	1935	5	10	NULL	NULL	NULL	Naphthalene cis-dihydrodiol	Chemical		bind					NDO	GP		active site		NULL		NULL	NULL	NULL	NULL	gw70_science_299_5609_1039_s_38	12586937	( D) Naphthalene  cis-dihydrodiol bound to the active site of NDO.	bind
3283	1	1935	7	10	NULL	NULL	NULL	Naphthalene cis-dihydrodiol	Chemical		bind					NDO	GP		active site of		NULL		NULL	NULL	NULL	NULL	gw70_science_299_5609_1039_s_38	12586937	( D) Naphthalene  cis-dihydrodiol bound to the active site of NDO.	bind
3653	1	1936	5	10	NULL	NULL	NULL	NAPQI-MIF	GP		bind					microvascular endothelial cells	Cell	human			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_1_144_s_167	11773615	( D) NAPQI-MIF shows decreased cell surface binding to human microvascular endothelial cells.	bind
3326	1	1936	7	10	NULL	NULL	NULL	NAPQI-MIF	GP		binds to					microvascular endothelial cell surface	Cell	human			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_1_144_s_167	11773615	( D) NAPQI-MIF shows decreased cell surface binding to human microvascular endothelial cells.	bind
3548	1	1937	5	10	NULL	NULL	NULL	Nef	GP		bind					cholesterol	Chemical				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_pnas_100_14_8460_s_210	12824470	( d) Nef binds  cholesterol  in vivo.	bind
3339	1	1937	7	10	NULL	NULL	NULL	Nef 	GP		bind					cholesterol	Chemical				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_pnas_100_14_8460_s_210	12824470	( d) Nef binds  cholesterol  in vivo.	bind
3554	1	1938	5	10	NULL	NULL	NULL	NF-IL6beta	GP		bind									C/EBP element	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_1_217_s_204	16397300	( D) NF-IL6beta binds to the C/EBP and CRE elements in DNA affinity precipitation assay.	bind
3555	2	1938	5	10	NULL	NULL	NULL	NF-IL6beta	GP		bind									CRE elements	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_1_217_s_204	16397300	( D) NF-IL6beta binds to the C/EBP and CRE elements in DNA affinity precipitation assay.	bind
3340	1	1938	7	10	NULL	NULL	NULL	NF-IL6beta 	GP		bind									C/EBP element	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_1_217_s_204	16397300	( D) NF-IL6beta binds to the C/EBP and CRE elements in DNA affinity precipitation assay.	bind
3341	2	1938	7	10	NULL	NULL	NULL	NF-IL6beta 	GP		bind									CRE element	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_1_217_s_204	16397300	( D) NF-IL6beta binds to the C/EBP and CRE elements in DNA affinity precipitation assay.	bind
5209	1	1939	5	10	NULL	NULL	NULL	NF-kappaB	GP		bind					DNA	NucleicAcid			single consensus Rel-binding site	NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10679_s_71	10485885	( d) NF-kappaB binds cooperatively with DSP1 to DNA bearing solely a single consensus Rel-binding site.	bind
5212	2	1939	5	10	NULL	NULL	NULL	DSP1	GP		bind					DNA	NucleicAcid			single consensus Rel-binding site	NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10679_s_71	10485885	( d) NF-kappaB binds cooperatively with DSP1 to DNA bearing solely a single consensus Rel-binding site.	bind
5213	3	1939	5	10	NULL	NULL	NULL	statement 1	Process		occurs in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10679_s_71	10485885	( d) NF-kappaB binds cooperatively with DSP1 to DNA bearing solely a single consensus Rel-binding site.	bind
3344	1	1939	7	10	NULL	NULL	NULL	NF-kappaB 	GP		bind					DNA	NucleicAcid			single consensus Rel-binding site	NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10679_s_71	10485885	( d) NF-kappaB binds cooperatively with DSP1 to DNA bearing solely a single consensus Rel-binding site.	bind
3345	2	1939	7	10	NULL	NULL	NULL	DSP1	GP		bind					DNA	NucleicAcid			single consensus Rel-binding site	NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10679_s_71	10485885	( d) NF-kappaB binds cooperatively with DSP1 to DNA bearing solely a single consensus Rel-binding site.	bind
4598	3	1939	7	10	NULL	NULL	NULL	statement 1	Process		occurs in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10679_s_71	10485885	( d) NF-kappaB binds cooperatively with DSP1 to DNA bearing solely a single consensus Rel-binding site.	bind
3655	1	1940	5	10	NULL	NULL	NULL	Ure2p	GP		bind					Gln3p	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_73_0_617_s_90	15189155	( D) Normally Ure2p binds the transcription factor Gln3p, preventing the upregulation  of genes, such as  DAL5, required for uptake of poor nitrogen sources.	bind
3656	2	1940	5	10	NULL	NULL	NULL	statement 1	Process		prevent					DAL5 gene	GP	upregulation of			NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_73_0_617_s_90	15189155	( D) Normally Ure2p binds the transcription factor Gln3p, preventing the upregulation  of genes, such as  DAL5, required for uptake of poor nitrogen sources.	bind
3657	3	1940	5	10	NULL	NULL	NULL	DAL5 gene	GP		is required for					poor nitrogen sources	Process	uptake of			NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_73_0_617_s_90	15189155	( D) Normally Ure2p binds the transcription factor Gln3p, preventing the upregulation  of genes, such as  DAL5, required for uptake of poor nitrogen sources.	bind
45663	4	1940	5	10	NULL	NULL	NULL	Gln3p	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_73_0_617_s_90	15189155	( D) Normally Ure2p binds the transcription factor Gln3p, preventing the upregulation  of genes, such as  DAL5, required for uptake of poor nitrogen sources.	bind
3346	1	1940	7	10	NULL	NULL	NULL	Ure2p	GP		bind					Gln3p	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_73_0_617_s_90	15189155	( D) Normally Ure2p binds the transcription factor Gln3p, preventing the upregulation  of genes, such as  DAL5, required for uptake of poor nitrogen sources.	bind
3347	2	1940	7	10	NULL	NULL	NULL	statement 1	Process		prevent					DAL5	GP	upregulation			NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_73_0_617_s_90	15189155	( D) Normally Ure2p binds the transcription factor Gln3p, preventing the upregulation  of genes, such as  DAL5, required for uptake of poor nitrogen sources.	bind
3348	3	1940	7	10	NULL	NULL	NULL	DAL5	GP		is required for					 poor nitrogen sources	Process	uptake of			NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_73_0_617_s_90	15189155	( D) Normally Ure2p binds the transcription factor Gln3p, preventing the upregulation  of genes, such as  DAL5, required for uptake of poor nitrogen sources.	bind
45665	4	1940	7	10	NULL	NULL	NULL	Gln3p	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_73_0_617_s_90	15189155	( D) Normally Ure2p binds the transcription factor Gln3p, preventing the upregulation  of genes, such as  DAL5, required for uptake of poor nitrogen sources.	bind
3658	1	1943	5	10	NULL	NULL	NULL	p25	GP		bind					STAT3	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_101_17_6728_s_100	15096606	( D) p25 binds STAT3  in vitro.	bind
3349	1	1943	7	10	NULL	NULL	NULL	 p25 	GP		binds					STAT3	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_101_17_6728_s_100	15096606	( D) p25 binds STAT3  in vitro.	bind
3659	1	1944	5	10	NULL	NULL	NULL	p52	GP		bind					Cyclin D1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_embo_25_20_4820_s_58	16990795	( D) p52 binds the Cyclin D1 promoter.	bind
3350	1	1944	7	10	NULL	NULL	NULL	p52	GP		bind					Cyclin D1 	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_embo_25_20_4820_s_58	16990795	( D) p52 binds the Cyclin D1 promoter.	bind
3660	1	1945	5	10	NULL	NULL	NULL	p53	GP		bind					MLH1	GP			p53RE	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_102_13_4813_s_132	15781865	( D) p53 binds to the MLH1 p53RE  in vitro.	bind
3351	1	1945	7	10	NULL	NULL	NULL	p53	GP		bind					MLH1	GP			p53RE	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_102_13_4813_s_132	15781865	( D) p53 binds to the MLH1 p53RE  in vitro.	bind
3661	1	1946	5	10	NULL	NULL	NULL	p65	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_25_10_1991_s_259	15192014	( D) p65 and H3 deacetylation is accompanied by inhibition of p65 binding to DNA. JB6  P+ cells were transfected with HDAC1 expression vector.	bind
3662	2	1946	5	10	NULL	NULL	NULL	p65	GP		undergoes					deacetylation	Process				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_25_10_1991_s_259	15192014	( D) p65 and H3 deacetylation is accompanied by inhibition of p65 binding to DNA. JB6  P+ cells were transfected with HDAC1 expression vector.	bind
3663	3	1946	5	10	NULL	NULL	NULL	H3	GP		undergoes					deacetylation	Process				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_25_10_1991_s_259	15192014	( D) p65 and H3 deacetylation is accompanied by inhibition of p65 binding to DNA. JB6  P+ cells were transfected with HDAC1 expression vector.	bind
50364	4	1946	5	10	NULL	NULL	NULL	statement 2	Process		is accompanied with					statement 1	Process	inhibition of 			NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_25_10_1991_s_259	15192014	( D) p65 and H3 deacetylation is accompanied by inhibition of p65 binding to DNA. JB6  P+ cells were transfected with HDAC1 expression vector.	bind
50365	5	1946	5	10	NULL	NULL	NULL	statement 3	Process		is accompanied with					statement 1	Process	inhibition of			NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_25_10_1991_s_259	15192014	( D) p65 and H3 deacetylation is accompanied by inhibition of p65 binding to DNA. JB6  P+ cells were transfected with HDAC1 expression vector.	bind
3352	1	1946	7	10	NULL	NULL	NULL	 p65 	GP		undergoes					deacetylation	Process				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_25_10_1991_s_259	15192014	( D) p65 and H3 deacetylation is accompanied by inhibition of p65 binding to DNA. JB6  P+ cells were transfected with HDAC1 expression vector.	bind
3353	2	1946	7	10	NULL	NULL	NULL	H3 	GP		undergoes					deacetylation	Process				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_25_10_1991_s_259	15192014	( D) p65 and H3 deacetylation is accompanied by inhibition of p65 binding to DNA. JB6  P+ cells were transfected with HDAC1 expression vector.	bind
3354	3	1946	7	10	NULL	NULL	NULL	p65	GP		binds					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_25_10_1991_s_259	15192014	( D) p65 and H3 deacetylation is accompanied by inhibition of p65 binding to DNA. JB6  P+ cells were transfected with HDAC1 expression vector.	bind
3355	4	1946	7	10	NULL	NULL	NULL	statement 1	Process		is accompanied with					statement 3	Process	inhibition of			NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_25_10_1991_s_259	15192014	( D) p65 and H3 deacetylation is accompanied by inhibition of p65 binding to DNA. JB6  P+ cells were transfected with HDAC1 expression vector.	bind
3356	5	1946	7	10	NULL	NULL	NULL	statement 2	Process		is accompanied with					statement 3	Process	inhibition of			NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_25_10_1991_s_259	15192014	( D) p65 and H3 deacetylation is accompanied by inhibition of p65 binding to DNA. JB6  P+ cells were transfected with HDAC1 expression vector.	bind
3664	1	1947	5	10	NULL	NULL	NULL	Mixer SIM peptide	GP		bind					Smad2	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_1_145_s_224	11782434	( D) Peptides corresponding to the Mixer SIM or to the SARA SBD peptide bind both Smad2 and phosphorylated Smad2, but only the SIM can bind a heteromeric complex of Smad2 and Smad4.	bind
3665	2	1947	5	10	NULL	NULL	NULL	Mixer SIM peptide	GP		bind					Smad2	GP	phosphorylated			NULL		NULL	NULL	NULL	NULL	gw60_embo_21_1_145_s_224	11782434	( D) Peptides corresponding to the Mixer SIM or to the SARA SBD peptide bind both Smad2 and phosphorylated Smad2, but only the SIM can bind a heteromeric complex of Smad2 and Smad4.	bind
3666	3	1947	5	10	NULL	NULL	NULL	SARA SBD peptide	GP		bind					Smad2	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_1_145_s_224	11782434	( D) Peptides corresponding to the Mixer SIM or to the SARA SBD peptide bind both Smad2 and phosphorylated Smad2, but only the SIM can bind a heteromeric complex of Smad2 and Smad4.	bind
3667	4	1947	5	10	NULL	NULL	NULL	SARA SBD peptide	GP		bind					Smad2	GP	phosphorylated			NULL		NULL	NULL	NULL	NULL	gw60_embo_21_1_145_s_224	11782434	( D) Peptides corresponding to the Mixer SIM or to the SARA SBD peptide bind both Smad2 and phosphorylated Smad2, but only the SIM can bind a heteromeric complex of Smad2 and Smad4.	bind
3668	5	1947	5	10	NULL	NULL	NULL	Smad2	GP		forms complex with					Smad4	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_1_145_s_224	11782434	( D) Peptides corresponding to the Mixer SIM or to the SARA SBD peptide bind both Smad2 and phosphorylated Smad2, but only the SIM can bind a heteromeric complex of Smad2 and Smad4.	bind
5214	6	1947	5	10	NULL	NULL	NULL	SIM	GP		bind					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_1_145_s_224	11782434	( D) Peptides corresponding to the Mixer SIM or to the SARA SBD peptide bind both Smad2 and phosphorylated Smad2, but only the SIM can bind a heteromeric complex of Smad2 and Smad4.	bind
3357	1	1947	7	10	NULL	NULL	NULL	Mixer SIM 	GP		bind					Smad2 	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_1_145_s_224	11782434	( D) Peptides corresponding to the Mixer SIM or to the SARA SBD peptide bind both Smad2 and phosphorylated Smad2, but only the SIM can bind a heteromeric complex of Smad2 and Smad4.	bind
3358	2	1947	7	10	NULL	NULL	NULL	Mixer SIM 	GP		bind					Smad2	GP	phosphorylated			NULL		NULL	NULL	NULL	NULL	gw60_embo_21_1_145_s_224	11782434	( D) Peptides corresponding to the Mixer SIM or to the SARA SBD peptide bind both Smad2 and phosphorylated Smad2, but only the SIM can bind a heteromeric complex of Smad2 and Smad4.	bind
3359	3	1947	7	10	NULL	NULL	NULL	SARA SBD peptide 	GP		bind					Smad2	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_1_145_s_224	11782434	( D) Peptides corresponding to the Mixer SIM or to the SARA SBD peptide bind both Smad2 and phosphorylated Smad2, but only the SIM can bind a heteromeric complex of Smad2 and Smad4.	bind
3360	4	1947	7	10	NULL	NULL	NULL	SARA SBD peptide 	GP		bind					Smad2	GP	phosphorylated 			NULL		NULL	NULL	NULL	NULL	gw60_embo_21_1_145_s_224	11782434	( D) Peptides corresponding to the Mixer SIM or to the SARA SBD peptide bind both Smad2 and phosphorylated Smad2, but only the SIM can bind a heteromeric complex of Smad2 and Smad4.	bind
3361	5	1947	7	10	NULL	NULL	NULL	Smad2	GP		forms complex with					Smad4	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_1_145_s_224	11782434	( D) Peptides corresponding to the Mixer SIM or to the SARA SBD peptide bind both Smad2 and phosphorylated Smad2, but only the SIM can bind a heteromeric complex of Smad2 and Smad4.	bind
3455	6	1947	7	10	NULL	NULL	NULL	SIM 	GP		bind					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_1_145_s_224	11782434	( D) Peptides corresponding to the Mixer SIM or to the SARA SBD peptide bind both Smad2 and phosphorylated Smad2, but only the SIM can bind a heteromeric complex of Smad2 and Smad4.	bind
3669	1	1948	5	10	NULL	NULL	NULL	PIP2	GP		bind					syntenin-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_14_2556_s_45	15961997	( D) PIP2 binding of syntenin-2 in overlay assay.	bind
3362	1	1948	7	10	NULL	NULL	NULL	PIP2	GP		bind					syntenin-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_14_2556_s_45	15961997	( D) PIP2 binding of syntenin-2 in overlay assay.	bind
3670	1	1949	5	10	NULL	NULL	NULL	PKNOX1	GP		bind		specifically							Pbx/POU target site	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_11_2769_s_175	12771203	( D) PKNOX1 binds specifically to the Pbx/POU target site and this binding is abolished  by the anti-PKNOX1 antibody.	bind
3671	2	1949	5	10	NULL	NULL	NULL	anti-PKNOX1 antibody	GP		abolish					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_11_2769_s_175	12771203	( D) PKNOX1 binds specifically to the Pbx/POU target site and this binding is abolished  by the anti-PKNOX1 antibody.	bind
3363	1	1949	7	10	NULL	NULL	NULL	PKNOX1	GP		binds		specifically							Pbx/POU target site 	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_11_2769_s_175	12771203	( D) PKNOX1 binds specifically to the Pbx/POU target site and this binding is abolished  by the anti-PKNOX1 antibody.	bind
3364	2	1949	7	10	NULL	NULL	NULL	statement 1	Process		is inhibited by					anti-PKNOX1 antibody	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_11_2769_s_175	12771203	( D) PKNOX1 binds specifically to the Pbx/POU target site and this binding is abolished  by the anti-PKNOX1 antibody.	bind
3672	1	1951	5	10	NULL	NULL	NULL	PTG	GP		bind					glycogen synthase	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_275_5305_1475_s_56	9045612	( D) PTG binds glycogen synthase.	bind
3365	1	1951	7	10	NULL	NULL	NULL	PTG 	GP		bind					glycogen synthase	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_275_5305_1475_s_56	9045612	( D) PTG binds glycogen synthase.	bind
3673	1	1952	5	10	NULL	NULL	NULL	MT	CellComponent		bind					KIF1A	GP	deletions			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1506_s_44	15014437	( D) Quantitative analysis of the MT binding (mean s.d.) of KIF1A deletions.	bind
4599	1	1952	7	10	NULL	NULL	NULL	MT	CellComponent		bind					KIF1A	GP	deletions of			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1506_s_44	15014437	( D) Quantitative analysis of the MT binding (mean s.d.) of KIF1A deletions.	bind
4032	1	1954	5	10	NULL	NULL	NULL	GATA-1	GP		bind					GATA- 2	GP			- 2.8 kb region of locus	NULL	untreated FOG-1 - / - cells	NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_102	14715908	( D) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to the  - 2.8 kb region  of  GATA- 2 locus in untreated and tamoxifen-treated (1muM, 24 h) FOG-1 - / -  and FOG-1 - / - -ER - GATA-1 cells (mean  plus-or-minus  SEM, five independent experiments).	bind
4033	2	1954	5	10	NULL	NULL	NULL	GATA-2	GP		bind					GATA- 2	GP			- 2.8 kb region of locus	NULL	untreated FOG-1 - / - cells	NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_102	14715908	( D) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to the  - 2.8 kb region  of  GATA- 2 locus in untreated and tamoxifen-treated (1muM, 24 h) FOG-1 - / -  and FOG-1 - / - -ER - GATA-1 cells (mean  plus-or-minus  SEM, five independent experiments).	bind
4034	3	1954	5	10	NULL	NULL	NULL	GATA-1	GP		bind					GATA- 2	GP			- 2.8 kb region of locus	NULL	tamoxifen-treated FOG-1 - / - cells	NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_102	14715908	( D) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to the  - 2.8 kb region  of  GATA- 2 locus in untreated and tamoxifen-treated (1muM, 24 h) FOG-1 - / -  and FOG-1 - / - -ER - GATA-1 cells (mean  plus-or-minus  SEM, five independent experiments).	bind
4035	4	1954	5	10	NULL	NULL	NULL	GATA-2	GP		bind					GATA- 2	GP			- 2.8 kb region of locus	NULL	tamoxifen-treated FOG-1 - / - cells	NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_102	14715908	( D) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to the  - 2.8 kb region  of  GATA- 2 locus in untreated and tamoxifen-treated (1muM, 24 h) FOG-1 - / -  and FOG-1 - / - -ER - GATA-1 cells (mean  plus-or-minus  SEM, five independent experiments).	bind
4253	5	1954	5	10	NULL	NULL	NULL	GATA-1	GP		bind					GATA- 2	GP			- 2.8 kb region of locus	NULL	untreated FOG-1 - / - -ER - GATA-1 cells	NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_102	14715908	( D) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to the  - 2.8 kb region  of  GATA- 2 locus in untreated and tamoxifen-treated (1muM, 24 h) FOG-1 - / -  and FOG-1 - / - -ER - GATA-1 cells (mean  plus-or-minus  SEM, five independent experiments).	bind
4254	6	1954	5	10	NULL	NULL	NULL	GATA-2	GP		bind					GATA- 2	GP			- 2.8 kb region of locus	NULL	untreated FOG-1 - / - -ER - GATA-1 cells	NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_102	14715908	( D) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to the  - 2.8 kb region  of  GATA- 2 locus in untreated and tamoxifen-treated (1muM, 24 h) FOG-1 - / -  and FOG-1 - / - -ER - GATA-1 cells (mean  plus-or-minus  SEM, five independent experiments).	bind
4255	7	1954	5	10	NULL	NULL	NULL	GATA-1	GP		bind					GATA- 2	GP			- 2.8 kb region of locus	NULL	tamoxifen-treated FOG-1 - / - -ER - GATA-1 cells	NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_102	14715908	( D) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to the  - 2.8 kb region  of  GATA- 2 locus in untreated and tamoxifen-treated (1muM, 24 h) FOG-1 - / -  and FOG-1 - / - -ER - GATA-1 cells (mean  plus-or-minus  SEM, five independent experiments).	bind
4256	8	1954	5	10	NULL	NULL	NULL	GATA-2	GP		bind					GATA- 2	GP			- 2.8 kb region of locus	NULL	tamoxifen-treated FOG-1 - / - -ER - GATA-1 cells	NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_102	14715908	( D) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to the  - 2.8 kb region  of  GATA- 2 locus in untreated and tamoxifen-treated (1muM, 24 h) FOG-1 - / -  and FOG-1 - / - -ER - GATA-1 cells (mean  plus-or-minus  SEM, five independent experiments).	bind
3366	1	1954	7	10	NULL	NULL	NULL	GATA-1	GP		binds to					GATA- 2 	GP	 		2.8 kb locus 	NULL	untreated FOG-1 - / - cells	NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_102	14715908	( D) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to the  - 2.8 kb region  of  GATA- 2 locus in untreated and tamoxifen-treated (1muM, 24 h) FOG-1 - / -  and FOG-1 - / - -ER - GATA-1 cells (mean  plus-or-minus  SEM, five independent experiments).	bind
3367	5	1954	7	10	NULL	NULL	NULL	GATA-2	GP		bind					GATA- 2	GP	 		2.8 kb  locus 	NULL	 untreated FOG-1 - / - cells	NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_102	14715908	( D) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to the  - 2.8 kb region  of  GATA- 2 locus in untreated and tamoxifen-treated (1muM, 24 h) FOG-1 - / -  and FOG-1 - / - -ER - GATA-1 cells (mean  plus-or-minus  SEM, five independent experiments).	bind
4602	2	1954	7	10	NULL	NULL	NULL	GATA-1	GP		bind					GATA- 2	GP	  		2.8 kb  locus	NULL	tamoxifen-treated FOG-1 - / - -ER - GATA-1 cells	NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_102	14715908	( D) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to the  - 2.8 kb region  of  GATA- 2 locus in untreated and tamoxifen-treated (1muM, 24 h) FOG-1 - / -  and FOG-1 - / - -ER - GATA-1 cells (mean  plus-or-minus  SEM, five independent experiments).	bind
4604	7	1954	7	10	NULL	NULL	NULL	GATA-2	GP		bind					GATA- 2 	GP	 		2.8 kb locus	NULL	tamoxifen-treated FOG-1 - / - -ER - GATA-1 cells	NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_102	14715908	( D) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to the  - 2.8 kb region  of  GATA- 2 locus in untreated and tamoxifen-treated (1muM, 24 h) FOG-1 - / -  and FOG-1 - / - -ER - GATA-1 cells (mean  plus-or-minus  SEM, five independent experiments).	bind
4607	3	1954	7	10	NULL	NULL	NULL	GATA-1	GP		bind					GATA- 2	GP			2.8 kb  locus	NULL	untreated FOG-1 - / - -ER - GATA-1 cells	NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_102	14715908	( D) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to the  - 2.8 kb region  of  GATA- 2 locus in untreated and tamoxifen-treated (1muM, 24 h) FOG-1 - / -  and FOG-1 - / - -ER - GATA-1 cells (mean  plus-or-minus  SEM, five independent experiments).	bind
4608	4	1954	7	10	NULL	NULL	NULL	GATA-1	GP		bind					GATA- 2	GP			2.8 kb  locus	NULL	tamoxifen-treated FOG-1 - / - cells	NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_102	14715908	( D) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to the  - 2.8 kb region  of  GATA- 2 locus in untreated and tamoxifen-treated (1muM, 24 h) FOG-1 - / -  and FOG-1 - / - -ER - GATA-1 cells (mean  plus-or-minus  SEM, five independent experiments).	bind
4609	6	1954	7	10	NULL	NULL	NULL	GATA-2 	GP		bind					GATA- 2 	GP			2.8 kb locus	NULL	untreated FOG-1 - / - -ER - GATA-1 cells 	NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_102	14715908	( D) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to the  - 2.8 kb region  of  GATA- 2 locus in untreated and tamoxifen-treated (1muM, 24 h) FOG-1 - / -  and FOG-1 - / - -ER - GATA-1 cells (mean  plus-or-minus  SEM, five independent experiments).	bind
4611	8	1954	7	10	NULL	NULL	NULL	GATA-2	GP		bind					 GATA- 2 	GP			2.8 kb locus	NULL	tamoxifen-treated FOG-1 - / - cells	NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_102	14715908	( D) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to the  - 2.8 kb region  of  GATA- 2 locus in untreated and tamoxifen-treated (1muM, 24 h) FOG-1 - / -  and FOG-1 - / - -ER - GATA-1 cells (mean  plus-or-minus  SEM, five independent experiments).	bind
4036	1	1955	5	10	NULL	NULL	NULL	GATA-1	GP		bind									GATA- 2 locus	NULL	FOG-1 - / - cells infected with empty vector	NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_142	14715908	( D) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to the  GATA- 2 locus in FOG-1 - / -  cells infected with empty or FOG-1-expressing retrovirus (mean  plus-or-minus  SEM  of five independent experiments).	bind
4037	2	1955	5	10	NULL	NULL	NULL	GATA-2	GP		bind									GATA- 2 locus	NULL	FOG-1 - / - cells infected with empty vector	NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_142	14715908	( D) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to the  GATA- 2 locus in FOG-1 - / -  cells infected with empty or FOG-1-expressing retrovirus (mean  plus-or-minus  SEM  of five independent experiments).	bind
4257	3	1955	5	10	NULL	NULL	NULL	GATA-1	GP		bind									GATA- 2 locus	NULL	FOG-1 - / - cells infected with FOG-1-expressing retrovirus	NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_142	14715908	( D) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to the  GATA- 2 locus in FOG-1 - / -  cells infected with empty or FOG-1-expressing retrovirus (mean  plus-or-minus  SEM  of five independent experiments).	bind
4258	4	1955	5	10	NULL	NULL	NULL	GATA-2	GP		bind									GATA- 2 locus	NULL	FOG-1 - / - cells infected with FOG-1-expressing retrovirus	NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_142	14715908	( D) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to the  GATA- 2 locus in FOG-1 - / -  cells infected with empty or FOG-1-expressing retrovirus (mean  plus-or-minus  SEM  of five independent experiments).	bind
3368	1	1955	7	10	NULL	NULL	NULL	GATA-1 	GP		bind									GATA- 2 locus 	NULL	 FOG-1 - / - cells infected with empty vector	NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_142	14715908	( D) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to the  GATA- 2 locus in FOG-1 - / -  cells infected with empty or FOG-1-expressing retrovirus (mean  plus-or-minus  SEM  of five independent experiments).	bind
3369	2	1955	7	10	NULL	NULL	NULL	GATA-2	GP		bind									GATA- 2 locus 	NULL	FOG-1 - / - cells infected with empty vector	NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_142	14715908	( D) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to the  GATA- 2 locus in FOG-1 - / -  cells infected with empty or FOG-1-expressing retrovirus (mean  plus-or-minus  SEM  of five independent experiments).	bind
46211	3	1955	7	10	NULL	NULL	NULL	 GATA-1	GP		bind									GATA- 2 locus	NULL	FOG-1 - / - cells infected with FOG-1-expressing retrovirus	NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_142	14715908	( D) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to the  GATA- 2 locus in FOG-1 - / -  cells infected with empty or FOG-1-expressing retrovirus (mean  plus-or-minus  SEM  of five independent experiments).	bind
46212	4	1955	7	10	NULL	NULL	NULL	GATA-2 	GP		bind									GATA- 2 locus	NULL	FOG-1 - / - cells infected with FOG-1-expressing retrovirus	NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_142	14715908	( D) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to the  GATA- 2 locus in FOG-1 - / -  cells infected with empty or FOG-1-expressing retrovirus (mean  plus-or-minus  SEM  of five independent experiments).	bind
4038	1	1956	5	10	NULL	NULL	NULL	GATA-2	GP		bind									GATA- 2 locus	NULL	G1E cells	NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_73	14715908	( D) Quantitative ChIP analysis of GATA-2 binding to the  GATA- 2 locus in G1E and FOG-1 - / -  cells (mean  plus-or-minus  SEM of three independent experiments).	bind
4259	2	1956	5	10	NULL	NULL	NULL	GATA-2	GP		bind									GATA- 2 locus	NULL	FOG-1 - / - cells	NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_73	14715908	( D) Quantitative ChIP analysis of GATA-2 binding to the  GATA- 2 locus in G1E and FOG-1 - / -  cells (mean  plus-or-minus  SEM of three independent experiments).	bind
3370	1	1956	7	10	NULL	NULL	NULL	GATA-2 	GP		bind					 				GATA- 2 locus	NULL	G1E cells 	NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_73	14715908	( D) Quantitative ChIP analysis of GATA-2 binding to the  GATA- 2 locus in G1E and FOG-1 - / -  cells (mean  plus-or-minus  SEM of three independent experiments).	bind
4620	2	1956	7	10	NULL	NULL	NULL	GATA-2	GP		bind									GATA- 2 locus	NULL	FOG-1 - / - cells	NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_73	14715908	( D) Quantitative ChIP analysis of GATA-2 binding to the  GATA- 2 locus in G1E and FOG-1 - / -  cells (mean  plus-or-minus  SEM of three independent experiments).	bind
3675	1	1957	5	10	NULL	NULL	NULL	Oct-1	GP		bind					 hIL2	GP			ARRE2 region in the promotor of	NULL		NULL	NULL	NULL	NULL	gw70_embo_25_5_1081_s_68	16498406	( D) Quantitative ChIP analysis was performed to determine the binding of Oct-1 and NFAT  and the modification of histone in the ARRE2 region of the  hIL2 promoter using real-time PCR.	bind
3676	2	1957	5	10	NULL	NULL	NULL	NFAT	GP		bind					hIL2	GP			ARRE2 region in the promotor of	NULL		NULL	NULL	NULL	NULL	gw70_embo_25_5_1081_s_68	16498406	( D) Quantitative ChIP analysis was performed to determine the binding of Oct-1 and NFAT  and the modification of histone in the ARRE2 region of the  hIL2 promoter using real-time PCR.	bind
5217	3	1957	5	10	NULL	NULL	NULL	histone	GP		is modified in					hIL2	GP			ARRE2 region in the promotor of	NULL		NULL	NULL	NULL	NULL	gw70_embo_25_5_1081_s_68	16498406	( D) Quantitative ChIP analysis was performed to determine the binding of Oct-1 and NFAT  and the modification of histone in the ARRE2 region of the  hIL2 promoter using real-time PCR.	bind
3371	1	1957	7	10	NULL	NULL	NULL	Oct-1	GP		bind					hIL2	GP			ARRE2 region in the promoter of	NULL		NULL	NULL	NULL	NULL	gw70_embo_25_5_1081_s_68	16498406	( D) Quantitative ChIP analysis was performed to determine the binding of Oct-1 and NFAT  and the modification of histone in the ARRE2 region of the  hIL2 promoter using real-time PCR.	bind
3372	2	1957	7	10	NULL	NULL	NULL	NFAT	GP		bind					hIL2 	GP			 ARRE2 region in the promoter of	NULL		NULL	NULL	NULL	NULL	gw70_embo_25_5_1081_s_68	16498406	( D) Quantitative ChIP analysis was performed to determine the binding of Oct-1 and NFAT  and the modification of histone in the ARRE2 region of the  hIL2 promoter using real-time PCR.	bind
4662	3	1957	7	10	NULL	NULL	NULL	histone	GP		is modified in					hIL2	GP			ARRE2 region in the promoter of	NULL		NULL	NULL	NULL	NULL	gw70_embo_25_5_1081_s_68	16498406	( D) Quantitative ChIP analysis was performed to determine the binding of Oct-1 and NFAT  and the modification of histone in the ARRE2 region of the  hIL2 promoter using real-time PCR.	bind
3677	1	1958	5	NULL	NULL	0	NULL	MDM2	NULL		bind	NULL				MDMX	NULL	different forms of			NULL	Saos2-MDMX cells	0	NULL	NULL	NULL	gw70_embo_24_19_3411_s_86	16163388	( D) Saos2-MDMX cells were tested for binding efficiencies of MDM2 to different forms  of MDMX by MDM2 IP and MDMX Western blot after irradiation in the presence of MG132.	bind
3678	2	1958	5	NULL	NULL	0	NULL	statement 1	NULL		in the presence of	NULL				MG132	NULL				NULL	Saos2-MDMX cells	NULL	NULL	NULL	NULL	gw70_embo_24_19_3411_s_86	16163388	( D) Saos2-MDMX cells were tested for binding efficiencies of MDM2 to different forms  of MDMX by MDM2 IP and MDMX Western blot after irradiation in the presence of MG132.	bind
3679	1	1959	5	10	NULL	NULL	NULL	Sema-2a-AP	GP		bind					S2R+ cells	Cell	PlexB-expressing			NULL		NULL	NULL	NULL	NULL	gw70_development_133_11_2125_s_239	16672342	( D) Scatchard analysis of Sema-2a-AP binding to PlexB-expressing S2R+ cells.	bind
3373	1	1959	7	10	NULL	NULL	NULL	Sema-2a-AP 	GP		bind					S2R+ cells	Cell	PlexB-expressing 			NULL		NULL	NULL	NULL	NULL	gw70_development_133_11_2125_s_239	16672342	( D) Scatchard analysis of Sema-2a-AP binding to PlexB-expressing S2R+ cells.	bind
3680	1	1960	5	10	NULL	NULL	NULL	AP-DCD	GP		bind					21NT breast cancer cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_19_10931_s_150	12953101	( D) Scatchard transformation of binding analysis of AP-DCD to 21NT breast cancer cells.	bind
3374	1	1960	7	10	NULL	NULL	NULL	AP-DCD 	GP		bind					21NT breast cancer cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_19_10931_s_150	12953101	( D) Scatchard transformation of binding analysis of AP-DCD to 21NT breast cancer cells.	bind
3681	1	1962	5	10	NULL	NULL	NULL	GST-PDZ1-2 fusion proteins	GP		bind					CFTR	GP		C terminus		NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_3_1300_s_140	11158634	( D) Sensorgram overlays for various GST-PDZ1-2 fusion proteins binding to CFTR C terminus at a concentration of 50 nM.	bind
3375	1	1962	7	10	NULL	NULL	NULL	GST-PDZ1-2 fusion proteins 	GP		bind					CFTR	GP		C terminus 		NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_3_1300_s_140	11158634	( D) Sensorgram overlays for various GST-PDZ1-2 fusion proteins binding to CFTR C terminus at a concentration of 50 nM.	bind
3682	1	1963	5	10	NULL	NULL	NULL	c-Jun	GP		bind					CSN5/Jab1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_7_1630_s_129	11285227	( D) Sequence alignment of the regions of c-Jun ( Claret  et al., 1996) and p27 Kip1 ( Tomoda  et al., 1999) that bind to CSN5/Jab1 with deltap53(1 - 154).	bind
3683	2	1963	5	10	NULL	NULL	NULL	p27 Kip1	GP		bind					 CSN5/Jab1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_7_1630_s_129	11285227	( D) Sequence alignment of the regions of c-Jun ( Claret  et al., 1996) and p27 Kip1 ( Tomoda  et al., 1999) that bind to CSN5/Jab1 with deltap53(1 - 154).	bind
3376	1	1963	7	10	NULL	NULL	NULL	c-Jun 	GP		bind					CSN5/Jab1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_7_1630_s_129	11285227	( D) Sequence alignment of the regions of c-Jun ( Claret  et al., 1996) and p27 Kip1 ( Tomoda  et al., 1999) that bind to CSN5/Jab1 with deltap53(1 - 154).	bind
3377	2	1963	7	10	NULL	NULL	NULL	p27 Kip1 	GP		bind					CSN5/Jab1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_7_1630_s_129	11285227	( D) Sequence alignment of the regions of c-Jun ( Claret  et al., 1996) and p27 Kip1 ( Tomoda  et al., 1999) that bind to CSN5/Jab1 with deltap53(1 - 154).	bind
3685	1	1964	5	10	NULL	NULL	NULL	Sid4p-myc	GP		bind		directly			Sid4deltaNp-HA	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_10_5249_s_192	10805785	( D) Sid4p-myc binds directly to Sid4deltaNp-HA.	bind
3379	1	1964	7	10	NULL	NULL	NULL	Sid4p-myc 	GP		binds		directly			Sid4deltaNp-HA	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_10_5249_s_192	10805785	( D) Sid4p-myc binds directly to Sid4deltaNp-HA.	bind
3686	1	1965	5	10	NULL	NULL	NULL	tubulin	GP	bovine	does not bind					GST-Aut7p glutathione-Sepharose 4B	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_13_3597_s_137	9649430	( D) Similar to (C), bovine tubulin does not bind to GST-Aut7p glutathione-Sepharose 4B (lane 12) and to GST glutathione-Sepharose 4B (lane 9).	bind
3687	2	1965	5	10	NULL	NULL	NULL	tubulin	GP	bovine	does not bind					GST glutathione-Sepharose 4B	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_13_3597_s_137	9649430	( D) Similar to (C), bovine tubulin does not bind to GST-Aut7p glutathione-Sepharose 4B (lane 12) and to GST glutathione-Sepharose 4B (lane 9).	bind
3380	1	1965	7	10	NULL	NULL	NULL	tubulin	GP	bovine	does not bind					GST-Aut7p glutathione-Sepharose 4B 	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_13_3597_s_137	9649430	( D) Similar to (C), bovine tubulin does not bind to GST-Aut7p glutathione-Sepharose 4B (lane 12) and to GST glutathione-Sepharose 4B (lane 9).	bind
3381	2	1965	7	10	NULL	NULL	NULL	tubulin	GP	bovine	does not bind					GST glutathione-Sepharose 4B 	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_13_3597_s_137	9649430	( D) Similar to (C), bovine tubulin does not bind to GST-Aut7p glutathione-Sepharose 4B (lane 12) and to GST glutathione-Sepharose 4B (lane 9).	bind
3688	1	1966	5	10	NULL	NULL	NULL	Sir1	GP		colocalize with					Ndc10	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_19_2356_s_50	12975325	( D) Sir1 colocalizes with centromere protein Ndc10.	bind
45677	2	1966	5	10	NULL	NULL	NULL	Ndc10	GP		is a type of					centromeric protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_19_2356_s_50	12975325	( D) Sir1 colocalizes with centromere protein Ndc10.	bind
3382	1	1966	7	10	NULL	NULL	NULL	Sir1	GP		colocalizes with					Ndc10 	GP		 		NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_19_2356_s_50	12975325	( D) Sir1 colocalizes with centromere protein Ndc10.	bind
45679	2	1966	7	10	NULL	NULL	NULL	Ndc10	GP		is a type of					centromeric protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_19_2356_s_50	12975325	( D) Sir1 colocalizes with centromere protein Ndc10.	bind
3689	1	1967	5	10	NULL	NULL	NULL	U1 snRNA	NucleicAcid		bind					SMN complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_5_1188_s_73	11867547	( D) SL1 domain of U1 snRNA is necessary for U1 snRNA binding of the SMN complex.	bind
3690	2	1967	5	10	NULL	NULL	NULL	U1 snRNA	NucleicAcid		is necessary for			SL1 domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_5_1188_s_73	11867547	( D) SL1 domain of U1 snRNA is necessary for U1 snRNA binding of the SMN complex.	bind
3383	1	1967	7	10	NULL	NULL	NULL	U1 snRNA 	NucleicAcid		binds to					 SMN complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_5_1188_s_73	11867547	( D) SL1 domain of U1 snRNA is necessary for U1 snRNA binding of the SMN complex.	bind
3384	2	1967	7	10	NULL	NULL	NULL	U1 snRNA 	NucleicAcid		is required for			SL1 domain 		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_5_1188_s_73	11867547	( D) SL1 domain of U1 snRNA is necessary for U1 snRNA binding of the SMN complex.	bind
3691	1	1968	5	10	NULL	NULL	NULL	Src	GP		bind					TRPV1	GP		proline-rich domain in the N-terminal region		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_24_4211_s_128	16319926	( D) Src binds to a proline-rich domain in the N-terminal region of TRPV1.	bind
3385	1	1968	7	10	NULL	NULL	NULL	 Src 	GP		bind					TRPV1	GP		proline-rich domain in the N-terminal region 		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_24_4211_s_128	16319926	( D) Src binds to a proline-rich domain in the N-terminal region of TRPV1.	bind
3692	1	1969	5	10	NULL	NULL	NULL	G1-Tbeta4	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_18_3599_s_88	15329672	( D) Stereo view of the structural overlap within the LKKTET-related motif between the  actin-bound forms of G1-Tbeta4 and ciboulot.	bind
3693	2	1969	5	10	NULL	NULL	NULL	ciboulot	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_18_3599_s_88	15329672	( D) Stereo view of the structural overlap within the LKKTET-related motif between the  actin-bound forms of G1-Tbeta4 and ciboulot.	bind
3386	1	1969	7	10	NULL	NULL	NULL	actin 	GP		bind					G1-Tbeta4 	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_18_3599_s_88	15329672	( D) Stereo view of the structural overlap within the LKKTET-related motif between the  actin-bound forms of G1-Tbeta4 and ciboulot.	bind
3387	2	1969	7	10	NULL	NULL	NULL	actin	GP		bind					ciboulot	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_18_3599_s_88	15329672	( D) Stereo view of the structural overlap within the LKKTET-related motif between the  actin-bound forms of G1-Tbeta4 and ciboulot.	bind
3694	1	1970	5	10	NULL	NULL	NULL	ThKaiCII peptide	GP		bind					ThKaiA	GP		C-terminal domains		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_9_2017_s_76	16628225	( D) Structural comparison between the NMR  ThKaiCII peptide bound to  ThKaiA C-terminal domains and the crystallographic model of the C-terminal end of the   SeKaiC A-chain: r.m.s. deviation 2.1  Ang .	bind
3389	1	1970	7	10	NULL	NULL	NULL	ThKaiCII peptide 	GP		bind					ThKaiA 	GP		C-terminal domains 		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_9_2017_s_76	16628225	( D) Structural comparison between the NMR  ThKaiCII peptide bound to  ThKaiA C-terminal domains and the crystallographic model of the C-terminal end of the   SeKaiC A-chain: r.m.s. deviation 2.1  Ang .	bind
3695	2	1971	5	10	NULL	NULL	NULL	Bcl-xL	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_21_0_35_s_131	16212486	( d) Structure of Bcl-xL bound to a BH3 peptide from Bad ( purple).	bind
46205	1	1971	5	10	NULL	NULL	NULL	BH3 peptide	GP		is derived from					Bad	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_21_0_35_s_131	16212486	( d) Structure of Bcl-xL bound to a BH3 peptide from Bad ( purple).	bind
3462	2	1971	7	10	NULL	NULL	NULL	Bcl-xL	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_21_0_35_s_131	16212486	( d) Structure of Bcl-xL bound to a BH3 peptide from Bad ( purple).	bind
46210	1	1971	7	10	NULL	NULL	NULL	BH3 peptide	GP		derived from					Bad	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_21_0_35_s_131	16212486	( d) Structure of Bcl-xL bound to a BH3 peptide from Bad ( purple).	bind
3696	1	1974	5	10	NULL	NULL	NULL	GST-eIF5	GP		bind					eIF2beta	GP		N		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_45_16164_s_115	16254050	( D) Summary of effects of eIF5 mutations, indicated to the right, on GST-eIF5 binding  to eIF2beta-N ( a), eIF3c-N ( b), and eIF1 ( c).	bind
3697	2	1974	5	10	NULL	NULL	NULL	GST-eIF5	GP		bind					eIF3c	GP		N		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_45_16164_s_115	16254050	( D) Summary of effects of eIF5 mutations, indicated to the right, on GST-eIF5 binding  to eIF2beta-N ( a), eIF3c-N ( b), and eIF1 ( c).	bind
3698	3	1974	5	10	NULL	NULL	NULL	GST-eIF5	GP		bind					eIF1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_45_16164_s_115	16254050	( D) Summary of effects of eIF5 mutations, indicated to the right, on GST-eIF5 binding  to eIF2beta-N ( a), eIF3c-N ( b), and eIF1 ( c).	bind
3481	1	1974	7	10	NULL	NULL	NULL	GST-eIF5	GP		bind					eIF2 beta	GP		N		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_45_16164_s_115	16254050	( D) Summary of effects of eIF5 mutations, indicated to the right, on GST-eIF5 binding  to eIF2beta-N ( a), eIF3c-N ( b), and eIF1 ( c).	bind
3482	2	1974	7	10	NULL	NULL	NULL	GST-eIF5	GP		bind					 eIF3c	GP		N		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_45_16164_s_115	16254050	( D) Summary of effects of eIF5 mutations, indicated to the right, on GST-eIF5 binding  to eIF2beta-N ( a), eIF3c-N ( b), and eIF1 ( c).	bind
3483	3	1974	7	10	NULL	NULL	NULL	GST-eIF5	GP		bind					eIF1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_45_16164_s_115	16254050	( D) Summary of effects of eIF5 mutations, indicated to the right, on GST-eIF5 binding  to eIF2beta-N ( a), eIF3c-N ( b), and eIF1 ( c).	bind
3699	1	1975	5	10	NULL	NULL	NULL	mt molecule	GP	nematode	bind					mt protein	GP	nematode			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_24_5444_s_177	12490713	( D) Summary of the binding specificities of nematode mt and bacterial EF-Tu molecules to nematode mt and bacterial EF-Ts proteins.	bind
3700	2	1975	5	10	NULL	NULL	NULL	mt molecule	GP	nematode	bind					EF-Ts protein	GP	bacterial			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_24_5444_s_177	12490713	( D) Summary of the binding specificities of nematode mt and bacterial EF-Tu molecules to nematode mt and bacterial EF-Ts proteins.	bind
3701	3	1975	5	10	NULL	NULL	NULL	EF-Tu molecule	GP	bacterial	bind					mt protein	GP	nematode			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_24_5444_s_177	12490713	( D) Summary of the binding specificities of nematode mt and bacterial EF-Tu molecules to nematode mt and bacterial EF-Ts proteins.	bind
3702	4	1975	5	10	NULL	NULL	NULL	EF-Tu molecule	GP	bacterial	bind					EF-Ts protein	GP	bacterial			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_24_5444_s_177	12490713	( D) Summary of the binding specificities of nematode mt and bacterial EF-Tu molecules to nematode mt and bacterial EF-Ts proteins.	bind
3484	1	1975	7	10	NULL	NULL	NULL	 mt  molecules	GP	nematode	bind					mt proteins	GP	nematode			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_24_5444_s_177	12490713	( D) Summary of the binding specificities of nematode mt and bacterial EF-Tu molecules to nematode mt and bacterial EF-Ts proteins.	bind
3485	2	1975	7	10	NULL	NULL	NULL	EF-Tu molecule	GP	bacterial	bind					EF-Ts proteins	GP	bacterial			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_24_5444_s_177	12490713	( D) Summary of the binding specificities of nematode mt and bacterial EF-Tu molecules to nematode mt and bacterial EF-Ts proteins.	bind
4227	3	1975	7	10	NULL	NULL	NULL	mt molecule	GP	nematode	bind					EF-Ts proteins	GP	bacterial			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_24_5444_s_177	12490713	( D) Summary of the binding specificities of nematode mt and bacterial EF-Tu molecules to nematode mt and bacterial EF-Ts proteins.	bind
4230	4	1975	7	10	NULL	NULL	NULL	EF-Tu molecule	GP	bacterial	bind					mt proteins	GP	nematode			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_24_5444_s_177	12490713	( D) Summary of the binding specificities of nematode mt and bacterial EF-Tu molecules to nematode mt and bacterial EF-Ts proteins.	bind
3703	1	1976	5	10	NULL	NULL	NULL	LEF1	GP	SUMO-modified	bind					beta-catenin	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_23_3088_s_190	11731474	( D) SUMO-modified LEF1 binds to beta-catenin.	bind
3486	1	1976	7	10	NULL	NULL	NULL	SUMO	GP		modifies					LEF1	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_23_3088_s_190	11731474	( D) SUMO-modified LEF1 binds to beta-catenin.	bind
3487	2	1976	7	10	NULL	NULL	NULL	statement 1	Process		bind					beta-catenin	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_23_3088_s_190	11731474	( D) SUMO-modified LEF1 binds to beta-catenin.	bind
3704	1	1977	5	10	NULL	NULL	NULL	pTP	GP		bind					Oct-1	GP	mutant	POUhd		NULL		NULL	NULL	NULL	NULL	gw60_embo_21_4_725_s_101	11847120	( D) Surface map of pTP binding by all identified Oct-1 POUhd mutants.	bind
3488	1	1977	7	10	NULL	NULL	NULL	pTP	GP		bind					Oct-1 	GP	mutants	POUhd		NULL		NULL	NULL	NULL	NULL	gw60_embo_21_4_725_s_101	11847120	( D) Surface map of pTP binding by all identified Oct-1 POUhd mutants.	bind
3705	1	1979	5	10	NULL	NULL	NULL	LIF	GP		induce					SOCS-3	GP	protein synthesis of			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_104_9_1277_s_224	10545526	( d) Sustained deactivation of LIF signaling also occurs through LIF-induced SOCS-3 protein synthesis and binding to JAK2, which appears maximally between 40 and 60 minutes of LIF stimulation.	bind
3706	2	1979	5	10	NULL	NULL	NULL	SOCS-3	GP		bind					JAK2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_104_9_1277_s_224	10545526	( d) Sustained deactivation of LIF signaling also occurs through LIF-induced SOCS-3 protein synthesis and binding to JAK2, which appears maximally between 40 and 60 minutes of LIF stimulation.	bind
3707	3	1979	5	10	NULL	NULL	NULL	LIF	GP		induce					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_104_9_1277_s_224	10545526	( d) Sustained deactivation of LIF signaling also occurs through LIF-induced SOCS-3 protein synthesis and binding to JAK2, which appears maximally between 40 and 60 minutes of LIF stimulation.	bind
3708	4	1979	5	10	NULL	NULL	NULL	LIF signaling	Process	deactivation of	occurs through					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_104_9_1277_s_224	10545526	( d) Sustained deactivation of LIF signaling also occurs through LIF-induced SOCS-3 protein synthesis and binding to JAK2, which appears maximally between 40 and 60 minutes of LIF stimulation.	bind
3709	5	1979	5	10	NULL	NULL	NULL	LIF signaling	Process	deactivation of	occurs through					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_104_9_1277_s_224	10545526	( d) Sustained deactivation of LIF signaling also occurs through LIF-induced SOCS-3 protein synthesis and binding to JAK2, which appears maximally between 40 and 60 minutes of LIF stimulation.	bind
3552	1	1979	7	10	NULL	NULL	NULL	LIF	GP		induce					SOCS-3	GP	protein synthesis of			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_104_9_1277_s_224	10545526	( d) Sustained deactivation of LIF signaling also occurs through LIF-induced SOCS-3 protein synthesis and binding to JAK2, which appears maximally between 40 and 60 minutes of LIF stimulation.	bind
3553	2	1979	7	10	NULL	NULL	NULL	SOCS-3	GP		binds to					JAK2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_104_9_1277_s_224	10545526	( d) Sustained deactivation of LIF signaling also occurs through LIF-induced SOCS-3 protein synthesis and binding to JAK2, which appears maximally between 40 and 60 minutes of LIF stimulation.	bind
3556	3	1979	7	10	NULL	NULL	NULL	statement 1	Process		cause					LIF signaling 	Process	 deactivation of			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_104_9_1277_s_224	10545526	( d) Sustained deactivation of LIF signaling also occurs through LIF-induced SOCS-3 protein synthesis and binding to JAK2, which appears maximally between 40 and 60 minutes of LIF stimulation.	bind
3940	4	1979	7	10	NULL	NULL	NULL	LIF	GP		induce					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_104_9_1277_s_224	10545526	( d) Sustained deactivation of LIF signaling also occurs through LIF-induced SOCS-3 protein synthesis and binding to JAK2, which appears maximally between 40 and 60 minutes of LIF stimulation.	bind
3941	5	1979	7	10	NULL	NULL	NULL	statement 4	Process		cause					LIF signaling 	Process	deactivation of			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_104_9_1277_s_224	10545526	( d) Sustained deactivation of LIF signaling also occurs through LIF-induced SOCS-3 protein synthesis and binding to JAK2, which appears maximally between 40 and 60 minutes of LIF stimulation.	bind
3739	1	1980	5	10	NULL	NULL	NULL	SXR:RXR heterodimers	GP		bind									IR-6 elements	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_20_3195_s_127	9784494	( D) SXR:RXR heterodimers bind to IR-6 elements.	bind
3489	1	1980	7	10	NULL	NULL	NULL	SXR:RXR	GP		binds to									IR-6	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_20_3195_s_127	9784494	( D) SXR:RXR heterodimers bind to IR-6 elements.	bind
3742	1	1981	5	10	NULL	NULL	NULL	synaptotagmin	GP		bind								mu2		NULL		NULL	NULL	NULL	NULL	gw60_embo_19_22_6011_s_46	11080148	( D) Synaptotagmin binds the mu2 and alpha subunits of disassembled AP-2.	bind
3808	2	1981	5	10	NULL	NULL	NULL	mu2	GP		is a subunit of					AP-2	GP	disassembled			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_22_6011_s_46	11080148	( D) Synaptotagmin binds the mu2 and alpha subunits of disassembled AP-2.	bind
3809	3	1981	5	10	NULL	NULL	NULL	synaptotagmin	GP		bind								alpha		NULL		NULL	NULL	NULL	NULL	gw60_embo_19_22_6011_s_46	11080148	( D) Synaptotagmin binds the mu2 and alpha subunits of disassembled AP-2.	bind
3810	4	1981	5	10	NULL	NULL	NULL	alpha	GP		is a subunit of					AP-2	GP	disassembled			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_22_6011_s_46	11080148	( D) Synaptotagmin binds the mu2 and alpha subunits of disassembled AP-2.	bind
3492	1	1981	7	10	NULL	NULL	NULL	Synaptotagmin 	GP		bind								mu2		NULL		NULL	NULL	NULL	NULL	gw60_embo_19_22_6011_s_46	11080148	( D) Synaptotagmin binds the mu2 and alpha subunits of disassembled AP-2.	bind
3493	2	1981	7	10	NULL	NULL	NULL	mu2	GP		is a subunit of					AP-2	GP	disassembled			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_22_6011_s_46	11080148	( D) Synaptotagmin binds the mu2 and alpha subunits of disassembled AP-2.	bind
3935	3	1981	7	10	NULL	NULL	NULL	Synaptotagmin	GP		bind								alpha		NULL		NULL	NULL	NULL	NULL	gw60_embo_19_22_6011_s_46	11080148	( D) Synaptotagmin binds the mu2 and alpha subunits of disassembled AP-2.	bind
3936	4	1981	7	10	NULL	NULL	NULL	alpha	GP		is a subunit of					AP-2	GP	disassembled			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_22_6011_s_46	11080148	( D) Synaptotagmin binds the mu2 and alpha subunits of disassembled AP-2.	bind
3744	1	1982	5	10	NULL	NULL	NULL	TFIIB	GP		bind					BNA1	GP			promoter	NULL	in vivo from WT mot1-42 cells	NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_153	15861138	( D) TFIIB binding to  BNA1 and  URA1 promoters  in vivo was determined by ChIP using chromatin from wild-type (WT) or  mot1-42 mutant cells.	bind
3745	3	1982	5	10	NULL	NULL	NULL	TFIIB	GP		bind					URA1	GP			promoter	NULL	in vivo from WT mot1-42 cells	NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_153	15861138	( D) TFIIB binding to  BNA1 and  URA1 promoters  in vivo was determined by ChIP using chromatin from wild-type (WT) or  mot1-42 mutant cells.	bind
46310	2	1982	5	10	NULL	NULL	NULL	TFIIB	GP		bind					BNA1	GP			promoter	NULL	in vivo from mot1-42 mutant cells	NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_153	15861138	( D) TFIIB binding to  BNA1 and  URA1 promoters  in vivo was determined by ChIP using chromatin from wild-type (WT) or  mot1-42 mutant cells.	bind
46311	4	1982	5	10	NULL	NULL	NULL	TFIIB	GP		bind					URA1	GP			promoter	NULL	in vivo from mot1-42 mutant cells	NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_153	15861138	( D) TFIIB binding to  BNA1 and  URA1 promoters  in vivo was determined by ChIP using chromatin from wild-type (WT) or  mot1-42 mutant cells.	bind
46312	5	1982	5	10	NULL	NULL	NULL	WT	Organism		is					wild-type	Organism				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_153	15861138	( D) TFIIB binding to  BNA1 and  URA1 promoters  in vivo was determined by ChIP using chromatin from wild-type (WT) or  mot1-42 mutant cells.	bind
3494	1	1982	7	10	NULL	NULL	NULL	TFIIB 	GP		bind					BNA1 	GP			promoter	NULL	in vivo from WT mot1-42  cells	NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_153	15861138	( D) TFIIB binding to  BNA1 and  URA1 promoters  in vivo was determined by ChIP using chromatin from wild-type (WT) or  mot1-42 mutant cells.	bind
3499	2	1982	7	10	NULL	NULL	NULL	TFIIB	GP		bind					BNA1	GP			promoter	NULL	in vivo from mot1-42 mutant cells	NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_153	15861138	( D) TFIIB binding to  BNA1 and  URA1 promoters  in vivo was determined by ChIP using chromatin from wild-type (WT) or  mot1-42 mutant cells.	bind
3500	3	1982	7	10	NULL	NULL	NULL	TFIIB	GP		bind					URA1	GP			promoter	NULL	in vivo from WT mot1-42  cells	NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_153	15861138	( D) TFIIB binding to  BNA1 and  URA1 promoters  in vivo was determined by ChIP using chromatin from wild-type (WT) or  mot1-42 mutant cells.	bind
46278	4	1982	7	10	NULL	NULL	NULL	TFIIB	GP		bind					URA1	GP			promoter	NULL	in vivo from mot1-42 mutant cells	NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_153	15861138	( D) TFIIB binding to  BNA1 and  URA1 promoters  in vivo was determined by ChIP using chromatin from wild-type (WT) or  mot1-42 mutant cells.	bind
46279	5	1982	7	10	NULL	NULL	NULL	WT	Organism		is					wild-type	Organism				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_153	15861138	( D) TFIIB binding to  BNA1 and  URA1 promoters  in vivo was determined by ChIP using chromatin from wild-type (WT) or  mot1-42 mutant cells.	bind
3746	1	1983	5	10	NULL	NULL	NULL	AKAP protein Yotiao	GP		bind					NMDA receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_9_1027_s_276	10809663	( D) The AKAP protein Yotiao binds to the NMDA receptor, PKA in the inactive form, and PP1 in the active form.	bind
3747	2	1983	5	10	NULL	NULL	NULL	AKAP protein Yotiao	GP		bind					PKA	GP	in inactive form			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_9_1027_s_276	10809663	( D) The AKAP protein Yotiao binds to the NMDA receptor, PKA in the inactive form, and PP1 in the active form.	bind
3748	3	1983	5	10	NULL	NULL	NULL	AKAP protein Yotiao	GP		bind					PP1	GP	in active form			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_9_1027_s_276	10809663	( D) The AKAP protein Yotiao binds to the NMDA receptor, PKA in the inactive form, and PP1 in the active form.	bind
3503	1	1983	7	10	NULL	NULL	NULL	AKAP protein Yotiao	GP		bind					NMDA receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_9_1027_s_276	10809663	( D) The AKAP protein Yotiao binds to the NMDA receptor, PKA in the inactive form, and PP1 in the active form.	bind
3506	2	1983	7	10	NULL	NULL	NULL	AKAP protein Yotiao	GP		binds to					PKA	GP	inactive form of 			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_9_1027_s_276	10809663	( D) The AKAP protein Yotiao binds to the NMDA receptor, PKA in the inactive form, and PP1 in the active form.	bind
3507	3	1983	7	10	NULL	NULL	NULL	AKAP protein Yotiao	GP		binds to					PP1	GP	active form of			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_9_1027_s_276	10809663	( D) The AKAP protein Yotiao binds to the NMDA receptor, PKA in the inactive form, and PP1 in the active form.	bind
3749	2	1984	5	10	NULL	NULL	NULL	Rad5p	GP		is not required for			ATP-binding motif		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_18_5878_s_41	16224103	( D) The ATP-binding motif of Rad5p is not required for polyubiquitylation of PCNA.	bind
46206	1	1984	5	10	NULL	NULL	NULL	PCNA	GP		undergoes					polyubiquitylation	Process				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_18_5878_s_41	16224103	( D) The ATP-binding motif of Rad5p is not required for polyubiquitylation of PCNA.	bind
3511	1	1984	7	10	NULL	NULL	NULL	PCNA	GP		undergoes					polyubiquitylation	Process				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_18_5878_s_41	16224103	( D) The ATP-binding motif of Rad5p is not required for polyubiquitylation of PCNA.	bind
3517	2	1984	7	10	NULL	NULL	NULL	Rad5p	GP		is not required for			ATP-binding motif		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_18_5878_s_41	16224103	( D) The ATP-binding motif of Rad5p is not required for polyubiquitylation of PCNA.	bind
3750	1	1985	5	10	NULL	NULL	NULL	ERK2	GP	mutant	bind					3pk	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_466_s_59	11157753	( D) The binding of the mutant forms of ERK2 to 3pk.	bind
3519	1	1985	7	10	NULL	NULL	NULL	ERK2	GP	mutant	bind					3pk	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_466_s_59	11157753	( D) The binding of the mutant forms of ERK2 to 3pk.	bind
3751	1	1986	5	10	NULL	NULL	NULL	ERK2	GP	mutant	bind					MSK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_466_s_287	11157753	( D) The binding of the mutant forms of ERK2 to MSK1 was examined as in	bind
3521	1	1986	7	10	NULL	NULL	NULL	ERK2	GP	mutant	bind					MSK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_466_s_287	11157753	( D) The binding of the mutant forms of ERK2 to MSK1 was examined as in	bind
3752	1	1987	5	10	NULL	NULL	NULL	p38	GP	mutant	bind					PRAK	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_466_s_237	11157753	( D) The binding of the mutant forms of p38 and ERK2 to PRAK was examined as in	bind
3753	2	1987	5	10	NULL	NULL	NULL	ERK2	GP	mutant	bind					PRAK	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_466_s_237	11157753	( D) The binding of the mutant forms of p38 and ERK2 to PRAK was examined as in	bind
3524	1	1987	7	10	NULL	NULL	NULL	p38	GP	mutant	bind 					PRAK	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_466_s_237	11157753	( D) The binding of the mutant forms of p38 and ERK2 to PRAK was examined as in	bind
3525	2	1987	7	10	NULL	NULL	NULL	ERK2	GP	mutant	bind					PRAK	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_466_s_237	11157753	( D) The binding of the mutant forms of p38 and ERK2 to PRAK was examined as in	bind
3754	1	1989	5	10	NULL	NULL	NULL	CREM factor	GP		bind					Oxct2b	GP			promoter	NULL	germ cell nuclei	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_10_3401_s_213	15951513	( D) The CREM factor binds to the Oxct2b promoter in germ cell nuclei.	bind
3526	1	1989	7	10	NULL	NULL	NULL	CREM factor	GP		bind					Oxct2b	GP			promoter	NULL	in germ cell nuclei	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_10_3401_s_213	15951513	( D) The CREM factor binds to the Oxct2b promoter in germ cell nuclei.	bind
3755	1	1991	5	10	NULL	NULL	NULL	dsDNA	NucleicAcid		bind					hRad54	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_6_1346_s_147	11884632	( D) The dsDNA binding of hRad54 and hRad54B.	bind
3756	2	1991	5	10	NULL	NULL	NULL	dsDNA	NucleicAcid		bind					hRad54B	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_6_1346_s_147	11884632	( D) The dsDNA binding of hRad54 and hRad54B.	bind
3527	1	1991	7	10	NULL	NULL	NULL	hRad54	GP		binds					dsDNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_6_1346_s_147	11884632	( D) The dsDNA binding of hRad54 and hRad54B.	bind
3529	2	1991	7	10	NULL	NULL	NULL	hRad54B	GP		binds					dsDNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_6_1346_s_147	11884632	( D) The dsDNA binding of hRad54 and hRad54B.	bind
4103	1	1992	5	10	NULL	NULL	NULL	kinase	GP		bind					E2F-1	GP		AD		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_15_4280_s_126	10428966	( D) The E2F-1 (AD)-bound kinase phosphorylates four substrates of TFIIH and the bound proteins comprise p62, p89 and cdk7.	bind
5223	2	1992	5	10	NULL	NULL	NULL	statement 1	Process		phosphorylate					four substrates of TFIIH	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_15_4280_s_126	10428966	( D) The E2F-1 (AD)-bound kinase phosphorylates four substrates of TFIIH and the bound proteins comprise p62, p89 and cdk7.	bind
3532	1	1992	7	10	NULL	NULL	NULL	kinase	GP		bind					E2F-1	GP		AD		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_15_4280_s_126	10428966	( D) The E2F-1 (AD)-bound kinase phosphorylates four substrates of TFIIH and the bound proteins comprise p62, p89 and cdk7.	bind
4664	2	1992	7	10	NULL	NULL	NULL	statement 1	Process		phosphorylates					four substrates of TFIIH 	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_15_4280_s_126	10428966	( D) The E2F-1 (AD)-bound kinase phosphorylates four substrates of TFIIH and the bound proteins comprise p62, p89 and cdk7.	bind
2602	1	1993	5	10	NULL	NULL	NULL	8-azido-[gamma-32]ATP	Chemical		bind					Kir6.2 proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_7_1318_s_55	15775962	( D) The IC50 values for Na-ATP competition of 8-azido-[gamma-32]ATP binding to Kir6.2 proteins confirms the synergistic effect of N- and C-terminal  interactions on nucleotide binding.	bind
2604	2	1993	5	10	NULL	NULL	NULL	Na-ATP	Chemical		bind					Kir6.2 proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_7_1318_s_55	15775962	( D) The IC50 values for Na-ATP competition of 8-azido-[gamma-32]ATP binding to Kir6.2 proteins confirms the synergistic effect of N- and C-terminal  interactions on nucleotide binding.	bind
3286	3	1993	5	10	NULL	NULL	NULL	statement 2	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_7_1318_s_55	15775962	( D) The IC50 values for Na-ATP competition of 8-azido-[gamma-32]ATP binding to Kir6.2 proteins confirms the synergistic effect of N- and C-terminal  interactions on nucleotide binding.	bind
3287	4	1993	5	10	NULL	NULL	NULL	N- and C-terminal interactions	Process		has synergistic effect on					nucleotide binding	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_7_1318_s_55	15775962	( D) The IC50 values for Na-ATP competition of 8-azido-[gamma-32]ATP binding to Kir6.2 proteins confirms the synergistic effect of N- and C-terminal  interactions on nucleotide binding.	bind
3288	5	1993	5	10	NULL	NULL	NULL	statement 3	Process		confirms					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_7_1318_s_55	15775962	( D) The IC50 values for Na-ATP competition of 8-azido-[gamma-32]ATP binding to Kir6.2 proteins confirms the synergistic effect of N- and C-terminal  interactions on nucleotide binding.	bind
3536	1	1993	7	10	NULL	NULL	NULL	8-azido-[gamma-32]ATP	Chemical		bind					Kir6.2 proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_7_1318_s_55	15775962	( D) The IC50 values for Na-ATP competition of 8-azido-[gamma-32]ATP binding to Kir6.2 proteins confirms the synergistic effect of N- and C-terminal  interactions on nucleotide binding.	bind
3537	2	1993	7	10	NULL	NULL	NULL	Na-ATP	Chemical		bind					Kir6.2 proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_7_1318_s_55	15775962	( D) The IC50 values for Na-ATP competition of 8-azido-[gamma-32]ATP binding to Kir6.2 proteins confirms the synergistic effect of N- and C-terminal  interactions on nucleotide binding.	bind
3539	4	1993	7	10	NULL	NULL	NULL	statement 1	Process		compete with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_7_1318_s_55	15775962	( D) The IC50 values for Na-ATP competition of 8-azido-[gamma-32]ATP binding to Kir6.2 proteins confirms the synergistic effect of N- and C-terminal  interactions on nucleotide binding.	bind
4231	5	1993	7	10	NULL	NULL	NULL	N- and C-terminal interactions 	Process		has synergistic effect on					nucleotide binding	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_7_1318_s_55	15775962	( D) The IC50 values for Na-ATP competition of 8-azido-[gamma-32]ATP binding to Kir6.2 proteins confirms the synergistic effect of N- and C-terminal  interactions on nucleotide binding.	bind
4232	6	1993	7	10	NULL	NULL	NULL	statement 4	Process		confirms					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_7_1318_s_55	15775962	( D) The IC50 values for Na-ATP competition of 8-azido-[gamma-32]ATP binding to Kir6.2 proteins confirms the synergistic effect of N- and C-terminal  interactions on nucleotide binding.	bind
2599	1	1995	5	10	NULL	NULL	NULL	MBS	GP		bind					moesin	GP		NH2-terminal domain		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_2_409_s_204	9548719	( D) The kinetic study of the MBS binding to the NH2-terminal domain  of moesin and the full-length moesin.	bind
2600	2	1995	5	10	NULL	NULL	NULL	MBS	GP		bind					moesin	GP	full-length			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_2_409_s_204	9548719	( D) The kinetic study of the MBS binding to the NH2-terminal domain  of moesin and the full-length moesin.	bind
3540	1	1995	7	10	NULL	NULL	NULL	MBS	GP		bind					moesin	GP		NH2-terminal domain 		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_2_409_s_204	9548719	( D) The kinetic study of the MBS binding to the NH2-terminal domain  of moesin and the full-length moesin.	bind
3541	2	1995	7	10	NULL	NULL	NULL	MBS	GP		bind					moesin	GP	full-length			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_2_409_s_204	9548719	( D) The kinetic study of the MBS binding to the NH2-terminal domain  of moesin and the full-length moesin.	bind
2594	1	1996	5	10	NULL	NULL	NULL	Ubc4(C/A)	GP		bind					pIkappaBalpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_15_4003_s_160	11483504	( D) The NEDD8 system does not support the binding of Ubc4(C/A) and Ubc4(C/S) to pIkappaBalpha.	bind
2596	2	1996	5	10	NULL	NULL	NULL	Ubc4(C/S)	GP		bind					pIkappaBalpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_15_4003_s_160	11483504	( D) The NEDD8 system does not support the binding of Ubc4(C/A) and Ubc4(C/S) to pIkappaBalpha.	bind
2597	3	1996	5	10	NULL	NULL	NULL	NEDD8 system	GP		does not support					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_15_4003_s_160	11483504	( D) The NEDD8 system does not support the binding of Ubc4(C/A) and Ubc4(C/S) to pIkappaBalpha.	bind
2598	4	1996	5	10	NULL	NULL	NULL	NEDD8 system	GP		does not support					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_15_4003_s_160	11483504	( D) The NEDD8 system does not support the binding of Ubc4(C/A) and Ubc4(C/S) to pIkappaBalpha.	bind
3542	1	1996	7	10	NULL	NULL	NULL	Ubc4(C/A)	GP		bind					pIkappaBalpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_15_4003_s_160	11483504	( D) The NEDD8 system does not support the binding of Ubc4(C/A) and Ubc4(C/S) to pIkappaBalpha.	bind
3543	2	1996	7	10	NULL	NULL	NULL	Ubc4(C/S)	GP		bind					pIkappaBalpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_15_4003_s_160	11483504	( D) The NEDD8 system does not support the binding of Ubc4(C/A) and Ubc4(C/S) to pIkappaBalpha.	bind
3544	3	1996	7	10	NULL	NULL	NULL	NEDD8 system	GP		does not support					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_15_4003_s_160	11483504	( D) The NEDD8 system does not support the binding of Ubc4(C/A) and Ubc4(C/S) to pIkappaBalpha.	bind
3545	4	1996	7	10	NULL	NULL	NULL	NEDD8 system	GP		does not support					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_15_4003_s_160	11483504	( D) The NEDD8 system does not support the binding of Ubc4(C/A) and Ubc4(C/S) to pIkappaBalpha.	bind
2590	1	1999	5	10	NULL	NULL	NULL	Cas	GP		bind					c-Crk	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_26_15394_s_91	9860979	( D) The substrate domain of Cas is required for Cas binding to c-Crk.	bind
2592	2	1999	5	10	NULL	NULL	NULL	Cas	GP		is required for			substrate domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_26_15394_s_91	9860979	( D) The substrate domain of Cas is required for Cas binding to c-Crk.	bind
3546	1	1999	7	10	NULL	NULL	NULL	 Cas	GP		bind					c-Crk	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_26_15394_s_91	9860979	( D) The substrate domain of Cas is required for Cas binding to c-Crk.	bind
3547	2	1999	7	10	NULL	NULL	NULL	Cas	GP		is required for			substrate domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_26_15394_s_91	9860979	( D) The substrate domain of Cas is required for Cas binding to c-Crk.	bind
2589	1	2000	5	10	NULL	0	NULL	serine	AminoAcid		bind					aMb-SerRS	GP		active site		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_11_2498_s_116	16675947	( D) The superposition of Ser-AMS, ATP and serine bound to the active site of aMb-SerRS.	bind
3289	2	2000	5	10	NULL	0	NULL	ATP	Chemical		bind					aMb-SerRS	GP		active site		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_11_2498_s_116	16675947	( D) The superposition of Ser-AMS, ATP and serine bound to the active site of aMb-SerRS.	bind
3290	3	2000	5	10	NULL	0	NULL	Ser-AMS	Chemical		bind					aMb-SerRS	GP		active site		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_11_2498_s_116	16675947	( D) The superposition of Ser-AMS, ATP and serine bound to the active site of aMb-SerRS.	bind
3549	1	2000	7	10	NULL	0	NULL	Ser-AMS	Chemical		binds to					aMb-SerRS	GP		active site of		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_11_2498_s_116	16675947	( D) The superposition of Ser-AMS, ATP and serine bound to the active site of aMb-SerRS.	bind
3550	2	2000	7	10	NULL	0	NULL	ATP	Chemical		binds to					aMb-SerRS	GP		active site of		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_11_2498_s_116	16675947	( D) The superposition of Ser-AMS, ATP and serine bound to the active site of aMb-SerRS.	bind
3551	3	2000	7	10	NULL	0	NULL	serine	AminoAcid		binds to					aMb-SerRS	GP		active site of		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_11_2498_s_116	16675947	( D) The superposition of Ser-AMS, ATP and serine bound to the active site of aMb-SerRS.	bind
2731	1	2001	6	10	NULL	0	NULL	TAK1	GP		bind					DR1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_32_14_4194_s_234	15302918	( D) TIP27 does not inhibit binding of TAK1 to DR1.	bind
2732	2	2001	6	10	NULL	0	NULL	TIP27	GP		does not inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_32_14_4194_s_234	15302918	( D) TIP27 does not inhibit binding of TAK1 to DR1.	bind
3557	1	2001	7	10	NULL	0	NULL	TAK1	GP		binds to					DR1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_32_14_4194_s_234	15302918	( D) TIP27 does not inhibit binding of TAK1 to DR1.	bind
3558	2	2001	7	10	NULL	0	NULL	TIP27 	GP		does not inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_32_14_4194_s_234	15302918	( D) TIP27 does not inhibit binding of TAK1 to DR1.	bind
2733	1	2002	6	10	NULL	0	NULL	TMEFF1	GP		bind		directly			Cripto coreceptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_21_2624_s_56	14563676	( D) TMEFF1 binds directly to the Cripto coreceptor.	bind
3559	1	2002	7	10	NULL	0	NULL	 TMEFF1	GP		binds		directly			Cripto coreceptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_21_2624_s_56	14563676	( D) TMEFF1 binds directly to the Cripto coreceptor.	bind
2738	1	2003	6	10	NULL	0	NULL	RA sera	CellComponent		bind					B7-H1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_111_3_363_s_94	12569162	( d) To examine specificity of RA sera binding to B7-H1, diluted sera were preincubated  with PBS, 2 mug/ml of soluble B7-H1Ig or control Ig (mIgG2a).	bind
3560	1	2003	7	10	NULL	0	NULL	RA sera	CellComponent		binds					B7-H1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_111_3_363_s_94	12569162	( d) To examine specificity of RA sera binding to B7-H1, diluted sera were preincubated  with PBS, 2 mug/ml of soluble B7-H1Ig or control Ig (mIgG2a).	bind
2739	1	2005	6	10	NULL	0	NULL	TRBP	GP		bind					TR	GP	liganded			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_pnas_97_11_6212_s_74	10823961	( D) TRBP binds to liganded TR and retinoic acid receptor (RAR)  in vitro.	bind
2740	2	2005	6	10	NULL	0	NULL	TRBP	GP		bind					RAR	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_pnas_97_11_6212_s_74	10823961	( D) TRBP binds to liganded TR and retinoic acid receptor (RAR)  in vitro.	bind
45776	3	2005	6	10	NULL	0	NULL	RAR	GP		is					retinoic acid receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_11_6212_s_74	10823961	( D) TRBP binds to liganded TR and retinoic acid receptor (RAR)  in vitro.	bind
3561	1	2005	7	10	NULL	0	NULL	TRBP	GP		binds to					TR	GP	liganded			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_pnas_97_11_6212_s_74	10823961	( D) TRBP binds to liganded TR and retinoic acid receptor (RAR)  in vitro.	bind
3562	2	2005	7	10	NULL	0	NULL	TRBP	GP		binds to					retinoic acid receptor 	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_pnas_97_11_6212_s_74	10823961	( D) TRBP binds to liganded TR and retinoic acid receptor (RAR)  in vitro.	bind
3563	3	2005	7	10	NULL	0	NULL	retinoic acid receptor	GP		is 					RAR	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_11_6212_s_74	10823961	( D) TRBP binds to liganded TR and retinoic acid receptor (RAR)  in vitro.	bind
2741	1	2006	6	10	NULL	0	NULL	COS-7 cells	Cell	live	express					VAB-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_2_187_s_86	12533508	( d) Two-hundred nanomolar MSP binds to the surface of live COS-7 cells (arrow) expressing VAB-1 ( upper panel), but not n-Src ( lower panel).	bind
2742	2	2006	6	10	NULL	0	NULL	MSP	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_2_187_s_86	12533508	( d) Two-hundred nanomolar MSP binds to the surface of live COS-7 cells (arrow) expressing VAB-1 ( upper panel), but not n-Src ( lower panel).	bind
2743	3	2006	6	10	NULL	0	NULL	COS-7 cells	Cell	live	express					n-Src	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_2_187_s_86	12533508	( d) Two-hundred nanomolar MSP binds to the surface of live COS-7 cells (arrow) expressing VAB-1 ( upper panel), but not n-Src ( lower panel).	bind
51547	4	2006	6	10	NULL	0	NULL	MSP	GP		does not bind					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_2_187_s_86	12533508	( d) Two-hundred nanomolar MSP binds to the surface of live COS-7 cells (arrow) expressing VAB-1 ( upper panel), but not n-Src ( lower panel).	bind
3564	1	2006	7	10	NULL	0	NULL	COS-7 cells	Cell	live	express					VAB-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_2_187_s_86	12533508	( d) Two-hundred nanomolar MSP binds to the surface of live COS-7 cells (arrow) expressing VAB-1 ( upper panel), but not n-Src ( lower panel).	bind
3565	2	2006	7	10	NULL	0	NULL	MSP	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_2_187_s_86	12533508	( d) Two-hundred nanomolar MSP binds to the surface of live COS-7 cells (arrow) expressing VAB-1 ( upper panel), but not n-Src ( lower panel).	bind
46265	3	2006	7	10	NULL	0	NULL	COS-7 cells	Cell	live	express					n-Src	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_2_187_s_86	12533508	( d) Two-hundred nanomolar MSP binds to the surface of live COS-7 cells (arrow) expressing VAB-1 ( upper panel), but not n-Src ( lower panel).	bind
46266	4	2006	7	10	NULL	0	NULL	MSP	GP		does not bind					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_2_187_s_86	12533508	( d) Two-hundred nanomolar MSP binds to the surface of live COS-7 cells (arrow) expressing VAB-1 ( upper panel), but not n-Src ( lower panel).	bind
2744	1	2007	6	10	NULL	0	NULL	c-Myc	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_14_8164_s_86	12808131	( D) Venn diagram comparing the DNA  binding of c-Myc and Max.	bind
2745	2	2007	6	10	NULL	0	NULL	Max	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_14_8164_s_86	12808131	( D) Venn diagram comparing the DNA  binding of c-Myc and Max.	bind
3566	1	2007	7	10	NULL	0	NULL	c-Myc	GP		binds					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_14_8164_s_86	12808131	( D) Venn diagram comparing the DNA  binding of c-Myc and Max.	bind
3567	2	2007	7	10	NULL	0	NULL	Max	GP		binds 					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_14_8164_s_86	12808131	( D) Venn diagram comparing the DNA  binding of c-Myc and Max.	bind
2748	1	2008	6	10	NULL	0	NULL	BCD	GP		bind					eIF4E	GP	recombinant			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_19_2576_s_37	12368268	( d) Western blots showing that BCD bound to m7GTP-sepharose coupled recombinant eIF4E (lanes  1,4) can be competed for with 100 nM (lane  2) and 1 mM (lanes  3,5) of a peptide containing the YDRKFL motif of human BP1, whereas 1 mM of a mutated human BP1 peptide (mutated motif is ADRKFR) did not interfere with the binding of BCD to eIF4E (lane  6).	bind
2750	2	2008	6	10	NULL	0	NULL	BP1	GP	human	bind			YDRKFL motif		e1F4E	GP	recombinant			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_19_2576_s_37	12368268	( d) Western blots showing that BCD bound to m7GTP-sepharose coupled recombinant eIF4E (lanes  1,4) can be competed for with 100 nM (lane  2) and 1 mM (lanes  3,5) of a peptide containing the YDRKFL motif of human BP1, whereas 1 mM of a mutated human BP1 peptide (mutated motif is ADRKFR) did not interfere with the binding of BCD to eIF4E (lane  6).	bind
2753	3	2008	6	10	NULL	0	NULL	BP1 peptide	GP	human;;mutant	does not interfere with			ADRKFR		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_19_2576_s_37	12368268	( d) Western blots showing that BCD bound to m7GTP-sepharose coupled recombinant eIF4E (lanes  1,4) can be competed for with 100 nM (lane  2) and 1 mM (lanes  3,5) of a peptide containing the YDRKFL motif of human BP1, whereas 1 mM of a mutated human BP1 peptide (mutated motif is ADRKFR) did not interfere with the binding of BCD to eIF4E (lane  6).	bind
5531	4	2008	6	10	NULL	0	NULL	statement 1	Process		competes with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_19_2576_s_37	12368268	( d) Western blots showing that BCD bound to m7GTP-sepharose coupled recombinant eIF4E (lanes  1,4) can be competed for with 100 nM (lane  2) and 1 mM (lanes  3,5) of a peptide containing the YDRKFL motif of human BP1, whereas 1 mM of a mutated human BP1 peptide (mutated motif is ADRKFR) did not interfere with the binding of BCD to eIF4E (lane  6).	bind
3572	1	2008	7	10	NULL	0	NULL	BCD	GP		binds to					eIF4E	GP	recombinant			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_19_2576_s_37	12368268	( d) Western blots showing that BCD bound to m7GTP-sepharose coupled recombinant eIF4E (lanes  1,4) can be competed for with 100 nM (lane  2) and 1 mM (lanes  3,5) of a peptide containing the YDRKFL motif of human BP1, whereas 1 mM of a mutated human BP1 peptide (mutated motif is ADRKFR) did not interfere with the binding of BCD to eIF4E (lane  6).	bind
3573	2	2008	7	10	NULL	0	NULL	 BP1	GP	human	binds to			YDRKFL motif		  eIF4E	GP	recombinant			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_19_2576_s_37	12368268	( d) Western blots showing that BCD bound to m7GTP-sepharose coupled recombinant eIF4E (lanes  1,4) can be competed for with 100 nM (lane  2) and 1 mM (lanes  3,5) of a peptide containing the YDRKFL motif of human BP1, whereas 1 mM of a mutated human BP1 peptide (mutated motif is ADRKFR) did not interfere with the binding of BCD to eIF4E (lane  6).	bind
3574	3	2008	7	10	NULL	0	NULL	BP1 peptide	GP	mutant;;human 	does not interfere with			ADRKFR motif		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_19_2576_s_37	12368268	( d) Western blots showing that BCD bound to m7GTP-sepharose coupled recombinant eIF4E (lanes  1,4) can be competed for with 100 nM (lane  2) and 1 mM (lanes  3,5) of a peptide containing the YDRKFL motif of human BP1, whereas 1 mM of a mutated human BP1 peptide (mutated motif is ADRKFR) did not interfere with the binding of BCD to eIF4E (lane  6).	bind
4233	4	2008	7	10	NULL	0	NULL	statement 1	Process		compete with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_19_2576_s_37	12368268	( d) Western blots showing that BCD bound to m7GTP-sepharose coupled recombinant eIF4E (lanes  1,4) can be competed for with 100 nM (lane  2) and 1 mM (lanes  3,5) of a peptide containing the YDRKFL motif of human BP1, whereas 1 mM of a mutated human BP1 peptide (mutated motif is ADRKFR) did not interfere with the binding of BCD to eIF4E (lane  6).	bind
2754	1	2009	6	10	NULL	0	NULL	Gal4 protein	GP	wild type	does not bind					Ubx	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_18_21_2596_s_40	15520279	( D) Wild-type GAL4 protein does not bind to the  Ubx promoter region.	bind
3568	1	2009	7	10	NULL	0	NULL	GAL4 protein	GP	Wild-type	does not bind					Ubx	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_18_21_2596_s_40	15520279	( D) Wild-type GAL4 protein does not bind to the  Ubx promoter region.	bind
2755	2	2010	6	10	NULL	0	NULL	XCdc6	GP		bind					statement 1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_2_472_s_243	10606645	( D) XCdc6 binds to the XORC-containing DNA.	bind
51548	1	2010	6	10	NULL	0	NULL	DNA	NucleicAcid		contains					XORC	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_2_472_s_243	10606645	( D) XCdc6 binds to the XORC-containing DNA.	bind
3569	2	2010	7	10	NULL	0	NULL	XCdc6	GP		bind					statement 1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_2_472_s_243	10606645	( D) XCdc6 binds to the XORC-containing DNA.	bind
46267	1	2010	7	10	NULL	0	NULL	DNA	NucleicAcid		contains					XORC	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_2_472_s_243	10606645	( D) XCdc6 binds to the XORC-containing DNA.	bind
2756	1	2011	6	10	NULL	0	NULL	synaptotagmin I 	GP		bind					AP-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_285_5431_1268_s_44	10455054	( D) YXX  peptides do not stimulate binding of synaptotagmin I to AP-1.	bind
3392	2	2011	6	10	NULL	0	NULL	YXX peptides	AminoAcid		does not stimulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_285_5431_1268_s_44	10455054	( D) YXX  peptides do not stimulate binding of synaptotagmin I to AP-1.	bind
3937	1	2011	7	10	NULL	0	NULL	synaptotagmin I	GP		bind to					AP-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_285_5431_1268_s_44	10455054	( D) YXX  peptides do not stimulate binding of synaptotagmin I to AP-1.	bind
3938	2	2011	7	10	NULL	0	NULL	YXX peptides	AminoAcid		do not stimulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_285_5431_1268_s_44	10455054	( D) YXX  peptides do not stimulate binding of synaptotagmin I to AP-1.	bind
2757	1	2012	6	10	NULL	0	NULL	ZF5	GP		bind		specifically						RRS motif		NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_26_14991_s_143	11734633	( D) ZF5 binds specifically to the RRS motif.	bind
3939	1	2012	7	10	NULL	0	NULL	ZF5	GP		binds		specifically						RRS motif		NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_26_14991_s_143	11734633	( D) ZF5 binds specifically to the RRS motif.	bind
2758	1	2013	6	10	NULL	0	NULL	Zip1	GP		bind					Pof1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_3_599_s_178	15660136	( D, E) Binding between Zip1 and Pof1.	bind
3942	1	2013	7	10	NULL	0	NULL	Zip1	GP		binds to					Pof1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_3_599_s_178	15660136	( D, E) Binding between Zip1 and Pof1.	bind
2759	1	2014	6	10	NULL	0	NULL	Robo2	GP	FLAG-tagged	bind			D1 5		Slit fragments	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_22_4406_s_75	15496984	( D, E) Binding of FLAG-tagged Robo2 D1 5 (D) and Robo3 D1 5 (E) to immobilised Slit fragments.	bind
2760	2	2014	6	10	NULL	0	NULL	Robo3	GP	FLAG-tagged	bind			D1 5		Slit fragments	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_22_4406_s_75	15496984	( D, E) Binding of FLAG-tagged Robo2 D1 5 (D) and Robo3 D1 5 (E) to immobilised Slit fragments.	bind
3943	1	2014	7	10	NULL	0	NULL	Robo2 	GP	FLAG-tagged	binds to			D1 5		Slit fragments	GP	immobilised			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_22_4406_s_75	15496984	( D, E) Binding of FLAG-tagged Robo2 D1 5 (D) and Robo3 D1 5 (E) to immobilised Slit fragments.	bind
3944	2	2014	7	10	NULL	0	NULL	Robo3 	GP	FLAG-tagged	binds to			D1 5		Slit fragments	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_22_4406_s_75	15496984	( D, E) Binding of FLAG-tagged Robo2 D1 5 (D) and Robo3 D1 5 (E) to immobilised Slit fragments.	bind
2996	1	2015	6	10	NULL	0	NULL	TIF32	GP		interacts with			NTD		RPS0A	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_6_786_s_302	12651896	( D,E) Hypothetical location of the eIF3 complex on the 3D model of the 40S subunit based  on the results of this study, including the requirements for the N- and C-terminal  domains in both NIP1 and TIF32 for 40S binding, interaction between the TIF32-NTD  and RPS0A, binding of the TIF32-CTD to helices 16-18 of 18S rRNA, and binding of  NIP1 to RPS0A and 18S rRNA.	bind
2997	2	2015	6	10	NULL	0	NULL	TIF32	GP		bind			CTD		18S rRNA	NucleicAcid			helices 16-18	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_6_786_s_302	12651896	( D,E) Hypothetical location of the eIF3 complex on the 3D model of the 40S subunit based  on the results of this study, including the requirements for the N- and C-terminal  domains in both NIP1 and TIF32 for 40S binding, interaction between the TIF32-NTD  and RPS0A, binding of the TIF32-CTD to helices 16-18 of 18S rRNA, and binding of  NIP1 to RPS0A and 18S rRNA.	bind
2998	3	2015	6	10	NULL	0	NULL	NIP1	GP		bind					RPS0A	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_6_786_s_302	12651896	( D,E) Hypothetical location of the eIF3 complex on the 3D model of the 40S subunit based  on the results of this study, including the requirements for the N- and C-terminal  domains in both NIP1 and TIF32 for 40S binding, interaction between the TIF32-NTD  and RPS0A, binding of the TIF32-CTD to helices 16-18 of 18S rRNA, and binding of  NIP1 to RPS0A and 18S rRNA.	bind
2999	4	2015	6	10	NULL	0	NULL	NIP1	GP		bind					18S rRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_6_786_s_302	12651896	( D,E) Hypothetical location of the eIF3 complex on the 3D model of the 40S subunit based  on the results of this study, including the requirements for the N- and C-terminal  domains in both NIP1 and TIF32 for 40S binding, interaction between the TIF32-NTD  and RPS0A, binding of the TIF32-CTD to helices 16-18 of 18S rRNA, and binding of  NIP1 to RPS0A and 18S rRNA.	bind
3000	5	2015	6	10	NULL	0	NULL	NIP1	GP		bind			N-terminal domain;;C-terminal domain		40S rRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_6_786_s_302	12651896	( D,E) Hypothetical location of the eIF3 complex on the 3D model of the 40S subunit based  on the results of this study, including the requirements for the N- and C-terminal  domains in both NIP1 and TIF32 for 40S binding, interaction between the TIF32-NTD  and RPS0A, binding of the TIF32-CTD to helices 16-18 of 18S rRNA, and binding of  NIP1 to RPS0A and 18S rRNA.	bind
3001	6	2015	6	10	NULL	0	NULL	TIF32	GP		bind			N-terminal domain;;C-terminal domain		40S rRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_6_786_s_302	12651896	( D,E) Hypothetical location of the eIF3 complex on the 3D model of the 40S subunit based  on the results of this study, including the requirements for the N- and C-terminal  domains in both NIP1 and TIF32 for 40S binding, interaction between the TIF32-NTD  and RPS0A, binding of the TIF32-CTD to helices 16-18 of 18S rRNA, and binding of  NIP1 to RPS0A and 18S rRNA.	bind
3945	1	2015	7	10	NULL	0	NULL	NIP1	GP		bind			N-terminal domain;;C-terminal domain		40S rRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_6_786_s_302	12651896	( D,E) Hypothetical location of the eIF3 complex on the 3D model of the 40S subunit based  on the results of this study, including the requirements for the N- and C-terminal  domains in both NIP1 and TIF32 for 40S binding, interaction between the TIF32-NTD  and RPS0A, binding of the TIF32-CTD to helices 16-18 of 18S rRNA, and binding of  NIP1 to RPS0A and 18S rRNA.	bind
3946	2	2015	7	10	NULL	0	NULL	TIF32	GP		bind			N-terminal domain;;C-terminal domain		40S rRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_6_786_s_302	12651896	( D,E) Hypothetical location of the eIF3 complex on the 3D model of the 40S subunit based  on the results of this study, including the requirements for the N- and C-terminal  domains in both NIP1 and TIF32 for 40S binding, interaction between the TIF32-NTD  and RPS0A, binding of the TIF32-CTD to helices 16-18 of 18S rRNA, and binding of  NIP1 to RPS0A and 18S rRNA.	bind
3947	3	2015	7	10	NULL	0	NULL	TIF32	GP		interacts with			NTD		RPS0A	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_6_786_s_302	12651896	( D,E) Hypothetical location of the eIF3 complex on the 3D model of the 40S subunit based  on the results of this study, including the requirements for the N- and C-terminal  domains in both NIP1 and TIF32 for 40S binding, interaction between the TIF32-NTD  and RPS0A, binding of the TIF32-CTD to helices 16-18 of 18S rRNA, and binding of  NIP1 to RPS0A and 18S rRNA.	bind
3948	4	2015	7	10	NULL	0	NULL	TIF32	GP		bind			CTD		18S rRNA	NucleicAcid			helices 16-18 of	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_6_786_s_302	12651896	( D,E) Hypothetical location of the eIF3 complex on the 3D model of the 40S subunit based  on the results of this study, including the requirements for the N- and C-terminal  domains in both NIP1 and TIF32 for 40S binding, interaction between the TIF32-NTD  and RPS0A, binding of the TIF32-CTD to helices 16-18 of 18S rRNA, and binding of  NIP1 to RPS0A and 18S rRNA.	bind
3949	5	2015	7	10	NULL	0	NULL	NIP1	GP		bind					RPS0A 	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_6_786_s_302	12651896	( D,E) Hypothetical location of the eIF3 complex on the 3D model of the 40S subunit based  on the results of this study, including the requirements for the N- and C-terminal  domains in both NIP1 and TIF32 for 40S binding, interaction between the TIF32-NTD  and RPS0A, binding of the TIF32-CTD to helices 16-18 of 18S rRNA, and binding of  NIP1 to RPS0A and 18S rRNA.	bind
3950	6	2015	7	10	NULL	0	NULL	NIP1	GP		bind					18S rRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_6_786_s_302	12651896	( D,E) Hypothetical location of the eIF3 complex on the 3D model of the 40S subunit based  on the results of this study, including the requirements for the N- and C-terminal  domains in both NIP1 and TIF32 for 40S binding, interaction between the TIF32-NTD  and RPS0A, binding of the TIF32-CTD to helices 16-18 of 18S rRNA, and binding of  NIP1 to RPS0A and 18S rRNA.	bind
2761	1	2017	6	10	NULL	0	NULL	Frat1	GP		bind					Dvl	GP				NULL	COS-7 cells	NULL	NULL	NULL	NULL	gw60_embo_18_15_4233_s_132	10428961	( D- F) Frat1 binds to Dvl in COS-7 cells.	bind
3951	1	2017	7	10	NULL	0	NULL	Frat1	GP		binds to					Dvl	GP				NULL	COS-7 cells	NULL	NULL	NULL	NULL	gw60_embo_18_15_4233_s_132	10428961	( D- F) Frat1 binds to Dvl in COS-7 cells.	bind
2763	1	2018	6	10	NULL	0	NULL	FGF2	GP		bind					FGFR2c	GP		S252W		NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_26_14536_s_147	11121055	( D-F) FGF2 binding to FGFR2c (S252W), FGFR2c (P253R), and FGFR2c, respectively.	bind
2765	2	2018	6	10	NULL	0	NULL	FGF2	GP		bind					FGFR2c	GP		P253R		NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_26_14536_s_147	11121055	( D-F) FGF2 binding to FGFR2c (S252W), FGFR2c (P253R), and FGFR2c, respectively.	bind
2766	3	2018	6	10	NULL	0	NULL	FGF2	GP		bind					FGFR2c	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_26_14536_s_147	11121055	( D-F) FGF2 binding to FGFR2c (S252W), FGFR2c (P253R), and FGFR2c, respectively.	bind
3952	1	2018	7	10	NULL	0	NULL	FGF2	GP		binds to					FGFR2c	GP		S252W		NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_26_14536_s_147	11121055	( D-F) FGF2 binding to FGFR2c (S252W), FGFR2c (P253R), and FGFR2c, respectively.	bind
3953	2	2018	7	10	NULL	0	NULL	FGF2	GP		binds to					FGFR2c	GP		P253R		NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_26_14536_s_147	11121055	( D-F) FGF2 binding to FGFR2c (S252W), FGFR2c (P253R), and FGFR2c, respectively.	bind
3954	3	2018	7	10	NULL	0	NULL	FGF2	GP		binds to					FGFR2c	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_26_14536_s_147	11121055	( D-F) FGF2 binding to FGFR2c (S252W), FGFR2c (P253R), and FGFR2c, respectively.	bind
2769	1	2019	6	10	NULL	0	NULL	AP-1	GP		bind					TGN	GP				NULL	mu1A-deficient cells	NULL	NULL	NULL	NULL	gw60_embo_19_10_2193_s_108	10811610	( E -  H) Binding of AP-1 to the TGN of control (E and H) and mu1A-deficient cells (F and G) permeabilized with digitonin.	bind
4234	1	2019	7	10	NULL	0	NULL	AP-1	GP		bind					TGN	GP				NULL	mu1A-deficient cells	NULL	NULL	NULL	NULL	gw60_embo_19_10_2193_s_108	10811610	( E -  H) Binding of AP-1 to the TGN of control (E and H) and mu1A-deficient cells (F and G) permeabilized with digitonin.	bind
2773	1	2021	6	10	NULL	0	NULL	F3 qdots	Chemical		bind					MDA-MB-435	Cell				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_20_12617_s_77	12235356	( e and  f) F3 qdots bind to MDA-MB-435 breast carcinoma cells ( e); free F3 peptide (500 muM) inhibits the binding ( f).	bind
2774	2	2021	6	10	NULL	0	NULL	MDA-MB-435	Cell		is a type of					breast carcinoma cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_20_12617_s_77	12235356	( e and  f) F3 qdots bind to MDA-MB-435 breast carcinoma cells ( e); free F3 peptide (500 muM) inhibits the binding ( f).	bind
2775	3	2021	6	10	NULL	0	NULL	F3 peptide	GP	free	inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_20_12617_s_77	12235356	( e and  f) F3 qdots bind to MDA-MB-435 breast carcinoma cells ( e); free F3 peptide (500 muM) inhibits the binding ( f).	bind
4235	1	2021	7	10	NULL	0	NULL	F3 qdots	Chemical		binds to					MDA-MB-435	Cell				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_20_12617_s_77	12235356	( e and  f) F3 qdots bind to MDA-MB-435 breast carcinoma cells ( e); free F3 peptide (500 muM) inhibits the binding ( f).	bind
4236	2	2021	7	10	NULL	0	NULL	 F3 peptide	GP	free	inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_20_12617_s_77	12235356	( e and  f) F3 qdots bind to MDA-MB-435 breast carcinoma cells ( e); free F3 peptide (500 muM) inhibits the binding ( f).	bind
45793	3	2021	7	10	NULL	0	NULL	MDA-MB-435	Cell		is a type of					breast carcinoma cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_20_12617_s_77	12235356	( e and  f) F3 qdots bind to MDA-MB-435 breast carcinoma cells ( e); free F3 peptide (500 muM) inhibits the binding ( f).	bind
2777	1	2022	6	10	NULL	0	NULL	LPC	Chemical		bind					G2A	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5530_702_s_63	11474113	( E and  F) Structural specificity of  [3]-16:0 LPC and [3]SPC  binding to G2A.	bind
2779	2	2022	6	10	NULL	0	NULL	SPC	Chemical		bind					G2A	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5530_702_s_63	11474113	( E and  F) Structural specificity of  [3]-16:0 LPC and [3]SPC  binding to G2A.	bind
4237	1	2022	7	10	NULL	0	NULL	LPC	Chemical		binds to					G2A	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5530_702_s_63	11474113	( E and  F) Structural specificity of  [3]-16:0 LPC and [3]SPC  binding to G2A.	bind
4238	2	2022	7	10	NULL	0	NULL	SPC	Chemical		binds to					G2A	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5530_702_s_63	11474113	( E and  F) Structural specificity of  [3]-16:0 LPC and [3]SPC  binding to G2A.	bind
2782	1	2023	6	10	NULL	0	NULL	MDMX	GP	in vitro translated	bind					GST-RB	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_5_2211_s_130	11226218	( E)  In vitro-translated MDMX binds to GST-RB and to GST-Sp1.	bind
2784	2	2023	6	10	NULL	0	NULL	MDMX	GP	in vitro translated	bind					GST-Sp1	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_5_2211_s_130	11226218	( E)  In vitro-translated MDMX binds to GST-RB and to GST-Sp1.	bind
4239	1	2023	7	10	NULL	0	NULL	MDMX	GP	in vitro-translated	binds to					GST-RB	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_5_2211_s_130	11226218	( E)  In vitro-translated MDMX binds to GST-RB and to GST-Sp1.	bind
4240	2	2023	7	10	NULL	0	NULL	MDMX	GP	in vitro-translated	binds to					GST-Sp1	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_5_2211_s_130	11226218	( E)  In vitro-translated MDMX binds to GST-RB and to GST-Sp1.	bind
2785	1	2024	6	10	NULL	0	NULL			hu6k array	bind				fraction of promotor or coding region	C-Myc	GP				NULL	Daudi cells	NULL	NULL	NULL	NULL	gw70_pnas_100_14_8164_s_90	12808131	( E) A comparison of the fraction of promoter  or coding regions represented on the hu6K  array that are bound by c-Myc, Max,  or both in Daudi cells.	bind
2786	2	2024	6	10	NULL	0	NULL			hu6k array	bind				fraction of promotor or coding region	Max	GP				NULL	Daudi cells	NULL	NULL	NULL	NULL	gw70_pnas_100_14_8164_s_90	12808131	( E) A comparison of the fraction of promoter  or coding regions represented on the hu6K  array that are bound by c-Myc, Max,  or both in Daudi cells.	bind
5787	3	2024	6	10	NULL	0	NULL	statement 1	Process		occur in conjunction with		may			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_14_8164_s_90	12808131	( E) A comparison of the fraction of promoter  or coding regions represented on the hu6K  array that are bound by c-Myc, Max,  or both in Daudi cells.	bind
4241	1	2024	7	10	NULL	0	NULL			hu6K array	bind				fraction of promoter or coding regions 	 c-Myc	GP				NULL	in Daudi cells	NULL	NULL	NULL	NULL	gw70_pnas_100_14_8164_s_90	12808131	( E) A comparison of the fraction of promoter  or coding regions represented on the hu6K  array that are bound by c-Myc, Max,  or both in Daudi cells.	bind
4242	2	2024	7	10	NULL	0	NULL			hu6K array	bind				fraction of promoter or coding regions 	Max	GP				NULL	in Daudi cells	NULL	NULL	NULL	NULL	gw70_pnas_100_14_8164_s_90	12808131	( E) A comparison of the fraction of promoter  or coding regions represented on the hu6K  array that are bound by c-Myc, Max,  or both in Daudi cells.	bind
4665	3	2024	7	10	NULL	0	NULL	statement 1	Process		occur in conjunction with		may			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_14_8164_s_90	12808131	( E) A comparison of the fraction of promoter  or coding regions represented on the hu6K  array that are bound by c-Myc, Max,  or both in Daudi cells.	bind
2795	1	2026	6	10	NULL	0	NULL	GFP-beta-CaMKII	GP	mutant	does not dissociate			A303R		F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5411_162_s_143	10102820	( E) A GFP-beta-CaMKII mutant deficient in calmodulin binding (A303R) fails to dissociate from F-actin after ionomycin addition.	bind
2796	2	2026	6	10	NULL	0	NULL	statement 1	Process		occurs after					ionomycin	Chemical	addition of			NULL		NULL	NULL	NULL	NULL	gw60_science_284_5411_162_s_143	10102820	( E) A GFP-beta-CaMKII mutant deficient in calmodulin binding (A303R) fails to dissociate from F-actin after ionomycin addition.	bind
5529	3	2026	6	10	NULL	0	NULL	CaMKII	GP	mutant	is deficient in			A303R		calmodulin	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_science_284_5411_162_s_143	10102820	( E) A GFP-beta-CaMKII mutant deficient in calmodulin binding (A303R) fails to dissociate from F-actin after ionomycin addition.	bind
4243	1	2026	7	10	NULL	0	NULL	GFP-beta-CaMKII 	GP	mutant	does not dissociate			A303R		F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5411_162_s_143	10102820	( E) A GFP-beta-CaMKII mutant deficient in calmodulin binding (A303R) fails to dissociate from F-actin after ionomycin addition.	bind
4244	2	2026	7	10	NULL	0	NULL	GFP-beta-CaMKII	GP	mutant	is deficient in			A303R		calmodulin 	GP	 binding of			NULL		NULL	NULL	NULL	NULL	gw60_science_284_5411_162_s_143	10102820	( E) A GFP-beta-CaMKII mutant deficient in calmodulin binding (A303R) fails to dissociate from F-actin after ionomycin addition.	bind
4245	3	2026	7	10	NULL	0	NULL	statement 1	Process		occurs after					ionomycin 	Chemical	addition of			NULL		NULL	NULL	NULL	NULL	gw60_science_284_5411_162_s_143	10102820	( E) A GFP-beta-CaMKII mutant deficient in calmodulin binding (A303R) fails to dissociate from F-actin after ionomycin addition.	bind
2797	1	2027	6	10	NULL	0	NULL	isocitrate	Chemical		bind					IDH1	GP		regulatory binding site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_15_12864_s_275	12562755	( E) A prerequisite for binding of AMP is binding of isocitrate by the IDH1 regulatory binding site.	bind
2798	2	2027	6	10	NULL	0	NULL	statement 1	Process		is prerequisite for					AMP	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_15_12864_s_275	12562755	( E) A prerequisite for binding of AMP is binding of isocitrate by the IDH1 regulatory binding site.	bind
4246	1	2027	7	10	NULL	0	NULL	IDH1 	GP		bind			regulatory binding site		isocitrate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_15_12864_s_275	12562755	( E) A prerequisite for binding of AMP is binding of isocitrate by the IDH1 regulatory binding site.	bind
4247	2	2027	7	10	NULL	0	NULL	statement 1	Process		is prerequisite					AMP	GP	for binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_15_12864_s_275	12562755	( E) A prerequisite for binding of AMP is binding of isocitrate by the IDH1 regulatory binding site.	bind
2799	1	2028	6	10	NULL	0	NULL	forskolin/TCDD-induced complex	GP		bind									DRE	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_26_9218_s_69	15972329	( E) AHR and ARNT proteins are present in the forskolin/TCDD-induced complex bound to  DRE.	bind
2800	2	2028	6	10	NULL	0	NULL	AHR protein	GP		present in					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_26_9218_s_69	15972329	( E) AHR and ARNT proteins are present in the forskolin/TCDD-induced complex bound to  DRE.	bind
2801	3	2028	6	10	NULL	0	NULL	ARNT protein	GP		present in					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_26_9218_s_69	15972329	( E) AHR and ARNT proteins are present in the forskolin/TCDD-induced complex bound to  DRE.	bind
4297	1	2028	7	10	NULL	0	NULL	forskolin/TCDD-induced complex	GP		bind									DRE	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_26_9218_s_69	15972329	( E) AHR and ARNT proteins are present in the forskolin/TCDD-induced complex bound to  DRE.	bind
4298	2	2028	7	10	NULL	0	NULL	AHR proteins	GP		 present in					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_26_9218_s_69	15972329	( E) AHR and ARNT proteins are present in the forskolin/TCDD-induced complex bound to  DRE.	bind
4299	3	2028	7	10	NULL	0	NULL	ARNT proteins	GP		 present in					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_26_9218_s_69	15972329	( E) AHR and ARNT proteins are present in the forskolin/TCDD-induced complex bound to  DRE.	bind
2802	1	2030	6	10	NULL	0	NULL	ASK1	GP		bind					AIP1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_111_12_1933_s_289	12813029	( e) ASK1 binding and the GAP activity of AIP1 are required for AIP1-enhanced ASK1 activation.	bind
2803	2	2030	6	10	NULL	0	NULL	AIP1	GP		activates					GAP	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_111_12_1933_s_289	12813029	( e) ASK1 binding and the GAP activity of AIP1 are required for AIP1-enhanced ASK1 activation.	bind
2804	4	2030	6	10	NULL	0	NULL	statement 1	Process		is required for					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_111_12_1933_s_289	12813029	( e) ASK1 binding and the GAP activity of AIP1 are required for AIP1-enhanced ASK1 activation.	bind
2805	5	2030	6	10	NULL	0	NULL	statement 2	Process		is required for					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_111_12_1933_s_289	12813029	( e) ASK1 binding and the GAP activity of AIP1 are required for AIP1-enhanced ASK1 activation.	bind
45805	3	2030	6	10	NULL	0	NULL	AIP1	GP		enhance					ASK1	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_111_12_1933_s_289	12813029	( e) ASK1 binding and the GAP activity of AIP1 are required for AIP1-enhanced ASK1 activation.	bind
4248	1	2030	7	10	NULL	0	NULL	ASK1	GP		bind					AIP1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_111_12_1933_s_289	12813029	( e) ASK1 binding and the GAP activity of AIP1 are required for AIP1-enhanced ASK1 activation.	bind
4249	2	2030	7	10	NULL	0	NULL	AIP1	Chemical		activates					GAP	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_111_12_1933_s_289	12813029	( e) ASK1 binding and the GAP activity of AIP1 are required for AIP1-enhanced ASK1 activation.	bind
4250	3	2030	7	10	NULL	0	NULL	AIP1	GP		enhance					ASK1	GP	activation of 			NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_111_12_1933_s_289	12813029	( e) ASK1 binding and the GAP activity of AIP1 are required for AIP1-enhanced ASK1 activation.	bind
4251	4	2030	7	10	NULL	0	NULL	statement 1	Process		is required for					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_111_12_1933_s_289	12813029	( e) ASK1 binding and the GAP activity of AIP1 are required for AIP1-enhanced ASK1 activation.	bind
4252	5	2030	7	10	NULL	0	NULL	statement 2	Process		is required for					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_111_12_1933_s_289	12813029	( e) ASK1 binding and the GAP activity of AIP1 are required for AIP1-enhanced ASK1 activation.	bind
2806	1	2031	6	10	NULL	0	NULL	Stat1	GP		associates 					Runx2	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_16_1979_s_184	12923053	( E) Association of Stat1 and Stat1CYF with Runx2 and the effect of  IFN-gamma on their phosphorylation and interaction.	bind
2807	2	2031	6	10	NULL	0	NULL	Stat1CYF	GP		associates 					Runx2	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_16_1979_s_184	12923053	( E) Association of Stat1 and Stat1CYF with Runx2 and the effect of  IFN-gamma on their phosphorylation and interaction.	bind
4300	1	2031	7	10	NULL	0	NULL	Stat1	GP		associate with					Runx2	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_16_1979_s_184	12923053	( E) Association of Stat1 and Stat1CYF with Runx2 and the effect of  IFN-gamma on their phosphorylation and interaction.	bind
4301	2	2031	7	10	NULL	0	NULL	Stat1CYF 	GP		associates with					Runx2	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_16_1979_s_184	12923053	( E) Association of Stat1 and Stat1CYF with Runx2 and the effect of  IFN-gamma on their phosphorylation and interaction.	bind
2808	1	2033	6	10	NULL	0	NULL	plasminogen	GP	125I-labeled	bind					ATP synthase	GP	human	alpha subunit		NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_6_2811_s_201	10077593	( E) Binding of 0.5 muM 125I-labeled plasminogen to the alpha-subunit of human ATP synthase.	bind
4306	1	2033	7	10	NULL	0	NULL	plasminogen	GP	125I-labeled	bind					ATP synthase	GP	human	alpha-subunit		NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_6_2811_s_201	10077593	( E) Binding of 0.5 muM 125I-labeled plasminogen to the alpha-subunit of human ATP synthase.	bind
2809	1	2034	6	10	NULL	0	NULL	EZI	GP	endogenous	bind					STAT3	GP	endogenous			NULL		NULL	NULL	NULL	NULL	gw60_embo_21_22_6174_s_120	12426389	( E) Binding of endogenous EZI and STAT3.	bind
4307	1	2034	7	10	NULL	0	NULL	 EZI	GP	endogenous	bind					STAT3	GP	endogenous			NULL		NULL	NULL	NULL	NULL	gw60_embo_21_22_6174_s_120	12426389	( E) Binding of endogenous EZI and STAT3.	bind
2810	1	2035	6	10	NULL	0	NULL	GST-beta1	GP		bind					mu2 constructs	GP		core domain (residues 283-394)		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_41_14871_s_111	16192353	( e) Binding of GST beta1 and beta3 to all constructs containing the core domain (residues 283-394) of mu2, whereas  GST-EGFR ( f), which contains a tyrosine type motif, binds to full length mu2	bind
2811	2	2035	6	10	NULL	0	NULL	GST-beta3	GP		bind					mu2 constructs	GP		core domain (residues 283-394)		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_41_14871_s_111	16192353	( e) Binding of GST beta1 and beta3 to all constructs containing the core domain (residues 283-394) of mu2, whereas  GST-EGFR ( f), which contains a tyrosine type motif, binds to full length mu2	bind
2812	3	2035	6	10	NULL	0	NULL	 GST-EGFR	GP		bind					mu2	GP	full length			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_41_14871_s_111	16192353	( e) Binding of GST beta1 and beta3 to all constructs containing the core domain (residues 283-394) of mu2, whereas  GST-EGFR ( f), which contains a tyrosine type motif, binds to full length mu2	bind
51549	3	2035	6	10	NULL	0	NULL	GST-EGFR	GP		contains								tyrosine type motif		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_41_14871_s_111	16192353	( e) Binding of GST beta1 and beta3 to all constructs containing the core domain (residues 283-394) of mu2, whereas  GST-EGFR ( f), which contains a tyrosine type motif, binds to full length mu2	bind
4308	1	2035	7	10	NULL	0	NULL	GST beta1	GP		bind					mu2 constructs	GP		core domain (residues 283-394)		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_41_14871_s_111	16192353	( e) Binding of GST beta1 and beta3 to all constructs containing the core domain (residues 283-394) of mu2, whereas  GST-EGFR ( f), which contains a tyrosine type motif, binds to full length mu2	bind
4309	2	2035	7	10	NULL	0	NULL	GST-beta3 	GP		bind					mu2 constructs	GP		core domain (residues 283-394)		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_41_14871_s_111	16192353	( e) Binding of GST beta1 and beta3 to all constructs containing the core domain (residues 283-394) of mu2, whereas  GST-EGFR ( f), which contains a tyrosine type motif, binds to full length mu2	bind
4310	3	2035	7	10	NULL	0	NULL	GST-EGFR	GP		bind					mu2	GP	full length 			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_41_14871_s_111	16192353	( e) Binding of GST beta1 and beta3 to all constructs containing the core domain (residues 283-394) of mu2, whereas  GST-EGFR ( f), which contains a tyrosine type motif, binds to full length mu2	bind
51550	4	2035	7	10	NULL	0	NULL	GST-EGFR	GP		contains								tyrosine type motif		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_41_14871_s_111	16192353	( e) Binding of GST beta1 and beta3 to all constructs containing the core domain (residues 283-394) of mu2, whereas  GST-EGFR ( f), which contains a tyrosine type motif, binds to full length mu2	bind
2813	1	2036	6	10	NULL	0	NULL	SF	GP	iodinated;;uncleavable	bind					A549	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_10_1418_s_61	15545993	( E) Binding of iodinated uncleavable SF to A549 human lung carcinoma cells.	bind
2814	2	2036	6	10	NULL	0	NULL	A549	Cell		is 					human lung carcinoma cells.	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_10_1418_s_61	15545993	( E) Binding of iodinated uncleavable SF to A549 human lung carcinoma cells.	bind
4311	1	2036	7	10	NULL	0	NULL	SF	GP	iodinated;;uncleavable	bind					A549	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_10_1418_s_61	15545993	( E) Binding of iodinated uncleavable SF to A549 human lung carcinoma cells.	bind
45806	2	2036	7	10	NULL	0	NULL	A549	Cell		is					human lung carcinoma cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_10_1418_s_61	15545993	( E) Binding of iodinated uncleavable SF to A549 human lung carcinoma cells.	bind
2815	1	2037	6	10	NULL	0	NULL	ORCA2	GP		bind					Str 	GP			RV fragment of promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_18_16_4455_s_152	10449411	( E) Binding of ORCA2 to the RV fragment of the  Str promoter.	bind
4312	1	2037	7	10	NULL	0	NULL	ORCA2	GP		bind					Str	GP			RV fragment of promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_18_16_4455_s_152	10449411	( E) Binding of ORCA2 to the RV fragment of the  Str promoter.	bind
2816	1	2038	6	10	NULL	0	NULL	p53	GP		bind					p38 kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_23_6845_s_97	10581258	( E) Binding of p53 and p38 kinase.	bind
4313	1	2038	7	10	NULL	0	NULL	p53	GP		bind					p38 kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_23_6845_s_97	10581258	( E) Binding of p53 and p38 kinase.	bind
2817	1	2039	6	10	NULL	0	NULL	PARP	GP		bind									cis-element	NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_1_48_s_177	11134536	( E) Binding of PARP to the  cis-element in GMSA.	bind
4314	1	2039	7	10	NULL	0	NULL	PARP	GP		bind									cis-element	NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_1_48_s_177	11134536	( E) Binding of PARP to the  cis-element in GMSA.	bind
2818	1	2040	6	10	NULL	0	NULL	CtBP	GP	recombinant	bind					GST-ZEB	GP		595-720		NULL		NULL	NULL	NULL	NULL	gw60_science_295_5561_1895_s_24	11847309	( E) Binding of recombinant CtBP to GST-ZEB595-720 at various concentrations of NAD+ and NADH.       [View Larger Version of this Image (76K GIF file)]	bind
4315	1	2040	7	10	NULL	0	NULL	CtBP	GP	recombinant	bind					GST-ZEB	GP		595-720		NULL		NULL	NULL	NULL	NULL	gw60_science_295_5561_1895_s_24	11847309	( E) Binding of recombinant CtBP to GST-ZEB595-720 at various concentrations of NAD+ and NADH.       [View Larger Version of this Image (76K GIF file)]	bind
2819	1	2041	6	10	NULL	0	NULL	IMP1	GP	recombinant	bind					CD44 mRNA	NucleicAcid			3'UTR 	NULL		NULL	NULL	NULL	NULL	gw70_embo_25_7_1456_s_227	16541107	( E) Binding of recombinant IMP1 to the 3'UTR of  CD44 mRNA.	bind
4316	1	2041	7	10	NULL	0	NULL	IMP1	GP	recombinant	bind					CD44 mRNA	NucleicAcid			 3'UTR 	NULL		NULL	NULL	NULL	NULL	gw70_embo_25_7_1456_s_227	16541107	( E) Binding of recombinant IMP1 to the 3'UTR of  CD44 mRNA.	bind
2886	1	2042	6	10	NULL	0	NULL	VDR	GP	recombinant	bind					DR3 oligonucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_7_2269_s_90	15849313	( E) Binding of recombinant VDR and RXR (100 ng) alone and in combination with the DR3  and DRE oligonucleotides.	bind
2887	2	2042	6	10	NULL	0	NULL	VDR	GP	recombinant	bind					DRE oligonucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_7_2269_s_90	15849313	( E) Binding of recombinant VDR and RXR (100 ng) alone and in combination with the DR3  and DRE oligonucleotides.	bind
2888	3	2042	6	10	NULL	0	NULL	RXR	GP	recombinant	bind					DR3 oligonucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_7_2269_s_90	15849313	( E) Binding of recombinant VDR and RXR (100 ng) alone and in combination with the DR3  and DRE oligonucleotides.	bind
2889	4	2042	6	10	NULL	0	NULL	RXR	GP	recombinant	bind					DRE oligonucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_7_2269_s_90	15849313	( E) Binding of recombinant VDR and RXR (100 ng) alone and in combination with the DR3  and DRE oligonucleotides.	bind
46180	5	2042	6	10	NULL	0	NULL	VDR-RXR	GP	recombinant	bind					DR3 oligonucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_7_2269_s_90	15849313	( E) Binding of recombinant VDR and RXR (100 ng) alone and in combination with the DR3  and DRE oligonucleotides.	bind
46181	6	2042	6	10	NULL	0	NULL	VDR-RXR	GP	recombinant	bind					DRE oligonucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_7_2269_s_90	15849313	( E) Binding of recombinant VDR and RXR (100 ng) alone and in combination with the DR3  and DRE oligonucleotides.	bind
4318	2	2042	7	10	NULL	0	NULL	VDR	GP	recombinant	binds					DR3 oligonucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_7_2269_s_90	15849313	( E) Binding of recombinant VDR and RXR (100 ng) alone and in combination with the DR3  and DRE oligonucleotides.	bind
4319	3	2042	7	10	NULL	0	NULL	VDR	GP	recombinant	binds					DRE oligonucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_7_2269_s_90	15849313	( E) Binding of recombinant VDR and RXR (100 ng) alone and in combination with the DR3  and DRE oligonucleotides.	bind
4666	4	2042	7	10	NULL	0	NULL	RXR	GP	recombinant	binds					DR3 oligonucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_7_2269_s_90	15849313	( E) Binding of recombinant VDR and RXR (100 ng) alone and in combination with the DR3  and DRE oligonucleotides.	bind
4667	5	2042	7	10	NULL	0	NULL	RXR	GP	recombinant	binds					DRE oligonucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_7_2269_s_90	15849313	( E) Binding of recombinant VDR and RXR (100 ng) alone and in combination with the DR3  and DRE oligonucleotides.	bind
46280	6	2042	7	10	NULL	0	NULL	VDR-RXR	GP	recombinant	bind					DR3 oligonucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_7_2269_s_90	15849313	( E) Binding of recombinant VDR and RXR (100 ng) alone and in combination with the DR3  and DRE oligonucleotides.	bind
46281	1	2042	7	10	NULL	0	NULL	VDR-RXR	GP	recombinant	bind					DRE oligonucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_7_2269_s_90	15849313	( E) Binding of recombinant VDR and RXR (100 ng) alone and in combination with the DR3  and DRE oligonucleotides.	bind
2890	1	2043	6	10	NULL	0	NULL	rML-LBP21	GP		bind					laminin alpha2 chain	GP		rG domain		NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_17_9857_s_189	10449784	( E) Binding of rML-LBP21 to the rG domain of laminin alpha2 chain in ELISA.	bind
4320	1	2043	7	10	NULL	0	NULL	rML-LBP21	GP		bind					laminin alpha2 chain	GP		 rG domain		NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_17_9857_s_189	10449784	( E) Binding of rML-LBP21 to the rG domain of laminin alpha2 chain in ELISA.	bind
2892	1	2045	6	10	NULL	0	NULL	FGF-7	GP	soluble	bind					perlecan	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_8_1599_s_189	9788974	( E) Binding of soluble FGF-7 to immobilized perlecan before and after heparitinase ( HSase) treatment.	bind
45807	2	2045	6	10	NULL	0	NULL	heparitinase \t	GP		is					HSase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_8_1599_s_189	9788974	( E) Binding of soluble FGF-7 to immobilized perlecan before and after heparitinase ( HSase) treatment.	bind
4323	1	2045	7	10	NULL	0	NULL	FGF-7	GP	soluble	bind					perlecan	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_8_1599_s_189	9788974	( E) Binding of soluble FGF-7 to immobilized perlecan before and after heparitinase ( HSase) treatment.	bind
4324	2	2045	7	10	NULL	0	NULL	heparitinase	GP		is					HSase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_8_1599_s_189	9788974	( E) Binding of soluble FGF-7 to immobilized perlecan before and after heparitinase ( HSase) treatment.	bind
2894	1	2046	6	10	NULL	0	NULL	sperm proteins	GP		bind					ZP	CellComponent	biotinylated			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_50_18028_s_154	16330764	( E) Binding of sperm proteins to biotinylated ZP.	bind
4325	1	2046	7	10	NULL	0	NULL	sperm proteins	GP		bind					ZP	CellComponent	biotinylated			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_50_18028_s_154	16330764	( E) Binding of sperm proteins to biotinylated ZP.	bind
2895	1	2047	6	10	NULL	0	NULL	TMEFF1	GP		bind					Cripto	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_21_2624_s_57	14563676	( E) Binding of TMEFF1 to Cripto reduces the association of ALK4 with Cripto.	bind
2896	2	2047	6	10	NULL	0	NULL	ALK4	GP		bind					Cripto	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_21_2624_s_57	14563676	( E) Binding of TMEFF1 to Cripto reduces the association of ALK4 with Cripto.	bind
2897	3	2047	6	10	NULL	0	NULL	statement 1	Process		reduces					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_21_2624_s_57	14563676	( E) Binding of TMEFF1 to Cripto reduces the association of ALK4 with Cripto.	bind
4326	1	2047	7	10	NULL	0	NULL	TMEFF1	GP		bind					Cripto	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_21_2624_s_57	14563676	( E) Binding of TMEFF1 to Cripto reduces the association of ALK4 with Cripto.	bind
4327	2	2047	7	10	NULL	0	NULL	 ALK4	GP		bind					Cripto	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_21_2624_s_57	14563676	( E) Binding of TMEFF1 to Cripto reduces the association of ALK4 with Cripto.	bind
4328	3	2047	7	10	NULL	0	NULL	statement 1	Process		reduce  					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_21_2624_s_57	14563676	( E) Binding of TMEFF1 to Cripto reduces the association of ALK4 with Cripto.	bind
2898	1	2049	6	10	NULL	0	NULL	rML-LBP21	GP		bind					alpha2-laminins	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_17_9857_s_51	10449784	( E) Characterization of rML-LBP21 binding to alpha2-laminins.	bind
4329	1	2049	7	10	NULL	0	NULL	rML-LBP21	GP		binds to					alpha2-laminins	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_17_9857_s_51	10449784	( E) Characterization of rML-LBP21 binding to alpha2-laminins.	bind
2909	1	2050	6	10	NULL	0	NULL	Pol II	GP		bind			delta5		c-myc 	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_16_5139_s_63	16157863	( E) ChIP analysis revealed similar binding of Pol II delta5 and Pol II wt to the c- myc promoter (lanes 3 and 11, respectively), while binding was not detectable in the  Mock cell line (lane 7), or ( F) to a non-transcribed region in the insulin gene.	bind
2910	2	2050	6	10	NULL	0	NULL	Pol II	GP	wt	bind					c-myc 	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_16_5139_s_63	16157863	( E) ChIP analysis revealed similar binding of Pol II delta5 and Pol II wt to the c- myc promoter (lanes 3 and 11, respectively), while binding was not detectable in the  Mock cell line (lane 7), or ( F) to a non-transcribed region in the insulin gene.	bind
2913	3	2050	6	10	NULL	0	NULL	statement 1	Process		is not detected in					Mock cell line	Cell				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_16_5139_s_63	16157863	( E) ChIP analysis revealed similar binding of Pol II delta5 and Pol II wt to the c- myc promoter (lanes 3 and 11, respectively), while binding was not detectable in the  Mock cell line (lane 7), or ( F) to a non-transcribed region in the insulin gene.	bind
2914	4	2050	6	10	NULL	0	NULL	statement 2	Process		is not detected in					Mock cell line	Cell				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_16_5139_s_63	16157863	( E) ChIP analysis revealed similar binding of Pol II delta5 and Pol II wt to the c- myc promoter (lanes 3 and 11, respectively), while binding was not detectable in the  Mock cell line (lane 7), or ( F) to a non-transcribed region in the insulin gene.	bind
2916	5	2050	6	10	NULL	0	NULL	statement 1	Process		is not detected in					insulin gene	GP			non transcribed region	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_16_5139_s_63	16157863	( E) ChIP analysis revealed similar binding of Pol II delta5 and Pol II wt to the c- myc promoter (lanes 3 and 11, respectively), while binding was not detectable in the  Mock cell line (lane 7), or ( F) to a non-transcribed region in the insulin gene.	bind
2917	6	2050	6	10	NULL	0	NULL	statement 2	Process		is not detected in					insulin gene	GP			non transcribed region	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_16_5139_s_63	16157863	( E) ChIP analysis revealed similar binding of Pol II delta5 and Pol II wt to the c- myc promoter (lanes 3 and 11, respectively), while binding was not detectable in the  Mock cell line (lane 7), or ( F) to a non-transcribed region in the insulin gene.	bind
4330	1	2050	7	10	NULL	0	NULL	Pol II 	GP		bind			delta5		c- myc	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_16_5139_s_63	16157863	( E) ChIP analysis revealed similar binding of Pol II delta5 and Pol II wt to the c- myc promoter (lanes 3 and 11, respectively), while binding was not detectable in the  Mock cell line (lane 7), or ( F) to a non-transcribed region in the insulin gene.	bind
4331	2	2050	7	10	NULL	0	NULL	Pol II	GP	wt	bind					c- myc	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_16_5139_s_63	16157863	( E) ChIP analysis revealed similar binding of Pol II delta5 and Pol II wt to the c- myc promoter (lanes 3 and 11, respectively), while binding was not detectable in the  Mock cell line (lane 7), or ( F) to a non-transcribed region in the insulin gene.	bind
4332	3	2050	7	10	NULL	0	NULL	statement 1	Process		not detected in					Mock cell line	Cell				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_16_5139_s_63	16157863	( E) ChIP analysis revealed similar binding of Pol II delta5 and Pol II wt to the c- myc promoter (lanes 3 and 11, respectively), while binding was not detectable in the  Mock cell line (lane 7), or ( F) to a non-transcribed region in the insulin gene.	bind
4333	4	2050	7	10	NULL	0	NULL	statement 2	Process		not detected in					Mock cell line	Cell				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_16_5139_s_63	16157863	( E) ChIP analysis revealed similar binding of Pol II delta5 and Pol II wt to the c- myc promoter (lanes 3 and 11, respectively), while binding was not detectable in the  Mock cell line (lane 7), or ( F) to a non-transcribed region in the insulin gene.	bind
4334	5	2050	7	10	NULL	0	NULL	statement 1	Process		not detected in					insulin gene	GP			non-transcribed region in	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_16_5139_s_63	16157863	( E) ChIP analysis revealed similar binding of Pol II delta5 and Pol II wt to the c- myc promoter (lanes 3 and 11, respectively), while binding was not detectable in the  Mock cell line (lane 7), or ( F) to a non-transcribed region in the insulin gene.	bind
4335	6	2050	7	10	NULL	0	NULL	statement 2	Process		not detected in					insulin gene	GP			non-transcribed region in	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_16_5139_s_63	16157863	( E) ChIP analysis revealed similar binding of Pol II delta5 and Pol II wt to the c- myc promoter (lanes 3 and 11, respectively), while binding was not detectable in the  Mock cell line (lane 7), or ( F) to a non-transcribed region in the insulin gene.	bind
2922	1	2051	6	10	NULL	0	NULL	CIITA	GP		bind					GTP	Chemical				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_science_285_5432_1402_s_62	10464099	( E) CIITA binds GTP in vivo.	bind
4336	1	2051	7	10	NULL	0	NULL	CIITA	GP		bind					GTP	Chemical				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_science_285_5432_1402_s_62	10464099	( E) CIITA binds GTP in vivo.	bind
2924	1	2052	6	10	NULL	0	NULL	Topotecan	GP		bind					enzyme-substrate complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_24_15387_s_71	12426403	( E) Comparison of the 22-mer duplex oligonucleotides of the drug-bound (blue) and nondrug-bound (yellow) complexes reveals that Topotecan (CPK) binds to the enzyme-substrate complex by intercalating in the DNA and shifting the downstream bases by  3.6  Ang , equivalent to the rise of one base pair.	bind
45808	2	2052	6	10	NULL	0	NULL	Topotecan	GP		is					CPK	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_24_15387_s_71	12426403	( E) Comparison of the 22-mer duplex oligonucleotides of the drug-bound (blue) and nondrug-bound (yellow) complexes reveals that Topotecan (CPK) binds to the enzyme-substrate complex by intercalating in the DNA and shifting the downstream bases by  3.6  Ang , equivalent to the rise of one base pair.	bind
4339	4	2052	7	10	NULL	0	NULL	Topotecan	GP		binds to					enzyme-substrate complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_24_15387_s_71	12426403	( E) Comparison of the 22-mer duplex oligonucleotides of the drug-bound (blue) and nondrug-bound (yellow) complexes reveals that Topotecan (CPK) binds to the enzyme-substrate complex by intercalating in the DNA and shifting the downstream bases by  3.6  Ang , equivalent to the rise of one base pair.	bind
4347	10	2052	7	10	NULL	0	NULL	Topotecan	GP		is					CPK	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_24_15387_s_71	12426403	( E) Comparison of the 22-mer duplex oligonucleotides of the drug-bound (blue) and nondrug-bound (yellow) complexes reveals that Topotecan (CPK) binds to the enzyme-substrate complex by intercalating in the DNA and shifting the downstream bases by  3.6  Ang , equivalent to the rise of one base pair.	bind
2925	1	2053	6	10	NULL	0	NULL	antihormones	Chemical	synthetic	bind					mPRgamma protein	GP	recombinant;;human			NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_5_2237_s_152	12601167	( e) Competition curves of binding of synthetic antihormones to the recombinant human mPRgamma protein.	bind
4348	1	2053	7	10	NULL	0	NULL	antihormones	Chemical	synthetic	binds to					mPRgamma protein	GP	recombinant;;human			NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_5_2237_s_152	12601167	( e) Competition curves of binding of synthetic antihormones to the recombinant human mPRgamma protein.	bind
2926	1	2054	6	10	NULL	0	NULL	GTP	Chemical		bind					Rac1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_111_8_1133_s_315	12697733	( e) Competition of GTP binding to Rac1 or Ras by 6-Thio-GTP.	bind
2927	2	2054	6	10	NULL	0	NULL	GTP	Chemical		bind					Ras	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_111_8_1133_s_315	12697733	( e) Competition of GTP binding to Rac1 or Ras by 6-Thio-GTP.	bind
2929	3	2054	6	10	NULL	0	NULL	6-Thio-GTP	Chemical		bind					Rac1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_111_8_1133_s_315	12697733	( e) Competition of GTP binding to Rac1 or Ras by 6-Thio-GTP.	bind
2930	4	2054	6	10	NULL	0	NULL	6-Thio-GTP	Chemical		bind					Ras	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_111_8_1133_s_315	12697733	( e) Competition of GTP binding to Rac1 or Ras by 6-Thio-GTP.	bind
3393	5	2054	6	10	NULL	0	NULL	statement 3	Process		competes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_111_8_1133_s_315	12697733	( e) Competition of GTP binding to Rac1 or Ras by 6-Thio-GTP.	bind
46329	6	2054	6	10	NULL	0	NULL	statement 4	Process		competes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_111_8_1133_s_315	12697733	( e) Competition of GTP binding to Rac1 or Ras by 6-Thio-GTP.	bind
4349	1	2054	7	10	NULL	0	NULL	GTP	Chemical		binds to					Rac1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_111_8_1133_s_315	12697733	( e) Competition of GTP binding to Rac1 or Ras by 6-Thio-GTP.	bind
4350	2	2054	7	10	NULL	0	NULL	GTP	Chemical		binds to					Ras	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_111_8_1133_s_315	12697733	( e) Competition of GTP binding to Rac1 or Ras by 6-Thio-GTP.	bind
4351	3	2054	7	10	NULL	0	NULL	6-Thio-GTP	Chemical		binds to					Rac1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_111_8_1133_s_315	12697733	( e) Competition of GTP binding to Rac1 or Ras by 6-Thio-GTP.	bind
4352	4	2054	7	10	NULL	0	NULL	6-Thio-GTP	Chemical		binds to					Ras	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_111_8_1133_s_315	12697733	( e) Competition of GTP binding to Rac1 or Ras by 6-Thio-GTP.	bind
4353	5	2054	7	10	NULL	0	NULL	statement 3	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_111_8_1133_s_315	12697733	( e) Competition of GTP binding to Rac1 or Ras by 6-Thio-GTP.	bind
4354	6	2054	7	10	NULL	0	NULL	statement 4	Process		compete with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_111_8_1133_s_315	12697733	( e) Competition of GTP binding to Rac1 or Ras by 6-Thio-GTP.	bind
2931	1	2055	6	10	NULL	0	NULL				bind			F-actin-binding domains		F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_26_14865_s_159	11752434	( E) Competitive binding of F-actin-binding domains to F-actin.	bind
4355	1	2055	7	10	NULL	0	NULL				binds to			F-actin-binding domains		F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_26_14865_s_159	11752434	( E) Competitive binding of F-actin-binding domains to F-actin.	bind
2932	1	2057	6	10	NULL	0	NULL	CHO cells	Cell		express					beta3	GP	WT			NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_43	12730600	( E) Constitutive fibrinogen binding to CHO cells expressing WT beta3 and the indicated beta3 mutants.	bind
2934	2	2057	6	10	NULL	0	NULL	CHO cells	Cell		express					beta3 	GP	mutants			NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_43	12730600	( E) Constitutive fibrinogen binding to CHO cells expressing WT beta3 and the indicated beta3 mutants.	bind
2935	3	2057	6	10	NULL	0	NULL	fibrinogen	GP		bind		constitutively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_43	12730600	( E) Constitutive fibrinogen binding to CHO cells expressing WT beta3 and the indicated beta3 mutants.	bind
2936	4	2057	6	10	NULL	0	NULL	fibrinogen	GP		bind		constitutively			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_43	12730600	( E) Constitutive fibrinogen binding to CHO cells expressing WT beta3 and the indicated beta3 mutants.	bind
4668	1	2057	7	10	NULL	0	NULL	CHO cells 	Cell		express					 beta3	GP	WT			NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_43	12730600	( E) Constitutive fibrinogen binding to CHO cells expressing WT beta3 and the indicated beta3 mutants.	bind
4669	2	2057	7	10	NULL	0	NULL	CHO cells	Cell		bind					beta3 	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_43	12730600	( E) Constitutive fibrinogen binding to CHO cells expressing WT beta3 and the indicated beta3 mutants.	bind
4670	3	2057	7	10	NULL	0	NULL	fibrinogen	GP		binds to		constitutively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_43	12730600	( E) Constitutive fibrinogen binding to CHO cells expressing WT beta3 and the indicated beta3 mutants.	bind
4671	4	2057	7	10	NULL	0	NULL	fibrinogen	GP		binds to		constitutively			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_43	12730600	( E) Constitutive fibrinogen binding to CHO cells expressing WT beta3 and the indicated beta3 mutants.	bind
2938	1	2058	6	10	NULL	0	NULL	CREB	GP		bind					nNOS	GP			CRE	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_15_8617_s_170	10900019	( E) CREB and ATF-2 bind to nNOS CRE.	bind
2940	2	2058	6	10	NULL	0	NULL	ATF-2	GP		bind					nNOS	GP			CRE	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_15_8617_s_170	10900019	( E) CREB and ATF-2 bind to nNOS CRE.	bind
4672	1	2058	7	10	NULL	0	NULL	CREB	GP		bind					nNOS	GP			CRE	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_15_8617_s_170	10900019	( E) CREB and ATF-2 bind to nNOS CRE.	bind
4673	2	2058	7	10	NULL	0	NULL	ATF-2 	GP		bind					nNOS	GP			CRE	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_15_8617_s_170	10900019	( E) CREB and ATF-2 bind to nNOS CRE.	bind
2941	1	2059	6	10	NULL	0	NULL	CTCF	GP		bind					Tsix	GP				NULL	in vivo female fibroblasts	NULL	NULL	NULL	NULL	gw60_science_295_5553_345_s_77	11743158	( E) CTCF binds  Tsix in vivo (female fibroblasts) using ChIP analysis as described ( 28).	bind
4674	1	2059	7	10	NULL	0	NULL	CTCF	GP		bind					 Tsix	GP				NULL	in vivo female fibroblasts	NULL	NULL	NULL	NULL	gw60_science_295_5553_345_s_77	11743158	( E) CTCF binds  Tsix in vivo (female fibroblasts) using ChIP analysis as described ( 28).	bind
2942	1	2060	6	10	NULL	0	NULL	DCX	GP		favors					13pf MTs	CellComponent	polymerization of			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_19_4448_s_61	16957770	( E) DCX favours polymerisation of 13pf MTs independent of the guanine nucleotide bound  to beta-tubulin.	bind
2944	2	2060	6	10	NULL	0	NULL	guanine nucleotide	NucleicAcid		bind					beta-tubulin	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_19_4448_s_61	16957770	( E) DCX favours polymerisation of 13pf MTs independent of the guanine nucleotide bound  to beta-tubulin.	bind
2945	3	2060	6	10	NULL	0	NULL	statement 1	Process		is independent of					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_19_4448_s_61	16957770	( E) DCX favours polymerisation of 13pf MTs independent of the guanine nucleotide bound  to beta-tubulin.	bind
4675	1	2060	7	10	NULL	0	NULL	DCX	GP		favours					13pf MTs	CellComponent	polymerisation of			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_19_4448_s_61	16957770	( E) DCX favours polymerisation of 13pf MTs independent of the guanine nucleotide bound  to beta-tubulin.	bind
4676	2	2060	7	10	NULL	0	NULL	guanine nucleotide	NucleicAcid		bind					beta-tubulin	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_19_4448_s_61	16957770	( E) DCX favours polymerisation of 13pf MTs independent of the guanine nucleotide bound  to beta-tubulin.	bind
4677	3	2060	7	10	NULL	0	NULL	statement 1	Process		is independent of					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_19_4448_s_61	16957770	( E) DCX favours polymerisation of 13pf MTs independent of the guanine nucleotide bound  to beta-tubulin.	bind
2946	1	2061	6	10	NULL	0	NULL	CREB	GP		bind					D-loop DNA	NucleicAcid	mitochondrial			NULL	in vivo in mouse primary cultures	NULL	NULL	NULL	NULL	gw70_pnas_102_39_13915_s_191	16169904	( E) DFO modulates  in vivo CREB binding to the mitochondrial D-loop DNA in mouse primary cultures.	bind
2949	2	2061	6	10	NULL	0	NULL	DFO	Chemical		modulates					statement 1	Process				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_pnas_102_39_13915_s_191	16169904	( E) DFO modulates  in vivo CREB binding to the mitochondrial D-loop DNA in mouse primary cultures.	bind
4679	1	2061	7	10	NULL	0	NULL	CREB	GP		binds to					D-loop DNA	NucleicAcid	mitochondrial			NULL	in vivo in mouse primary cultures	NULL	NULL	NULL	NULL	gw70_pnas_102_39_13915_s_191	16169904	( E) DFO modulates  in vivo CREB binding to the mitochondrial D-loop DNA in mouse primary cultures.	bind
4680	2	2061	7	10	NULL	0	NULL	DFO	Chemical		modulates					statement 1	Process				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_pnas_102_39_13915_s_191	16169904	( E) DFO modulates  in vivo CREB binding to the mitochondrial D-loop DNA in mouse primary cultures.	bind
2952	1	2062	6	10	NULL	0	NULL	TLX	GP		bind		directly			Plce1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_20_10_1308_s_217	16702404	( E) Direct binding of TLX to the  Plce1 promoter was determined by gel shift assays as described in Figure  6F.	bind
4681	1	2062	7	10	NULL	0	NULL	TLX	GP		binds		directly			Plce1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_20_10_1308_s_217	16702404	( E) Direct binding of TLX to the  Plce1 promoter was determined by gel shift assays as described in Figure  6F.	bind
2961	1	2063	6	10	NULL	0	NULL	fusion proteins	GP		bind			GST-PDZ domain		synaptojanin 2A 	GP		C-terminal peptide		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_11_2991_s_80	10357812	( E) Dose-response curves of binding of GST-PDZ domain fusion proteins to the synaptojanin 2A C-terminal peptide in an ELISA assay.	bind
4682	1	2063	7	10	NULL	0	NULL	fusion proteins	GP		binds			GST-PDZ domain		synaptojanin 2A	GP		C-terminal peptide		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_11_2991_s_80	10357812	( E) Dose-response curves of binding of GST-PDZ domain fusion proteins to the synaptojanin 2A C-terminal peptide in an ELISA assay.	bind
2962	1	2064	6	10	NULL	0	NULL	Ecsit 2	GP		bind					Tlx2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_23_2933_s_249	14633973	( E) Ecsit 2, Smad1, and Smad4 bind to the  Tlx2 promoter.	bind
2963	2	2064	6	10	NULL	0	NULL	Smad1	GP		bind					Tlx2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_23_2933_s_249	14633973	( E) Ecsit 2, Smad1, and Smad4 bind to the  Tlx2 promoter.	bind
2964	3	2064	6	10	NULL	0	NULL	Smad4	GP		bind					Tlx2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_23_2933_s_249	14633973	( E) Ecsit 2, Smad1, and Smad4 bind to the  Tlx2 promoter.	bind
4685	1	2064	7	10	NULL	0	NULL	Ecsit 2	GP		binds					Tlx2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_23_2933_s_249	14633973	( E) Ecsit 2, Smad1, and Smad4 bind to the  Tlx2 promoter.	bind
4687	2	2064	7	10	NULL	0	NULL	Smad1	GP		binds					Tlx2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_23_2933_s_249	14633973	( E) Ecsit 2, Smad1, and Smad4 bind to the  Tlx2 promoter.	bind
4688	3	2064	7	10	NULL	0	NULL	Smad4	GP		binds					Tlx2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_23_2933_s_249	14633973	( E) Ecsit 2, Smad1, and Smad4 bind to the  Tlx2 promoter.	bind
2991	1	2065	6	10	NULL	0	NULL	AP-1	GP		bind									CRE	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_29_10194_s_61	16000406	( E) Effect of CHX on AP-1 and CRE binding.	bind
4690	1	2065	7	10	NULL	0	NULL	AP-1	GP		binds									CRE	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_29_10194_s_61	16000406	( E) Effect of CHX on AP-1 and CRE binding.	bind
2992	1	2066	6	10	NULL	0	NULL	E2F4	GP		bind					c-myc 	GP			promoter	NULL	C2C12 cells	NULL	NULL	NULL	NULL	gw60_pnas_100_6_3245_s_124	12629224	( E) Effects of lithium stimulation on binding of E2F4, p130, and HDAC1 to the c- Myc promoter in C2C12 cells.	bind
2993	2	2066	6	10	NULL	0	NULL	p130	GP		bind					c-myc 	GP			promoter	NULL	C2C12 cells	NULL	NULL	NULL	NULL	gw60_pnas_100_6_3245_s_124	12629224	( E) Effects of lithium stimulation on binding of E2F4, p130, and HDAC1 to the c- Myc promoter in C2C12 cells.	bind
2994	3	2066	6	10	NULL	0	NULL	HDAC1	GP		bind					c-myc 	GP			promoter	NULL	C2C12 cells	NULL	NULL	NULL	NULL	gw60_pnas_100_6_3245_s_124	12629224	( E) Effects of lithium stimulation on binding of E2F4, p130, and HDAC1 to the c- Myc promoter in C2C12 cells.	bind
4695	1	2066	7	10	NULL	0	NULL	E2F4	GP		binds					 c- Myc	GP			promoter	NULL	in C2C12 cells	NULL	NULL	NULL	NULL	gw60_pnas_100_6_3245_s_124	12629224	( E) Effects of lithium stimulation on binding of E2F4, p130, and HDAC1 to the c- Myc promoter in C2C12 cells.	bind
4696	2	2066	7	10	NULL	0	NULL	p130	GP		binds					 c- Myc	GP			promoter	NULL	in C2C12 cells	NULL	NULL	NULL	NULL	gw60_pnas_100_6_3245_s_124	12629224	( E) Effects of lithium stimulation on binding of E2F4, p130, and HDAC1 to the c- Myc promoter in C2C12 cells.	bind
4697	3	2066	7	10	NULL	0	NULL	HDAC1	GP		binds					c- myc	GP			promoter	NULL	in C2C12 cells	NULL	NULL	NULL	NULL	gw60_pnas_100_6_3245_s_124	12629224	( E) Effects of lithium stimulation on binding of E2F4, p130, and HDAC1 to the c- Myc promoter in C2C12 cells.	bind
2995	1	2067	6	10	NULL	0	NULL	Emi1	GP		bind					Cdc20	GP		SBR		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_24_3278_s_110	11751633	( E) Emi1 binds the substrate-binding region (SBR) of Cdc20.	bind
3394	2	2067	6	10	NULL	0	NULL	SBR	AminoAcid		is					substrate-binding region	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_24_3278_s_110	11751633	( E) Emi1 binds the substrate-binding region (SBR) of Cdc20.	bind
4699	1	2067	7	10	NULL	0	NULL	Emi1	GP		binds					Cdc20	GP		SBR		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_24_3278_s_110	11751633	( E) Emi1 binds the substrate-binding region (SBR) of Cdc20.	bind
4700	2	2067	7	10	NULL	0	NULL	SBR	AminoAcid		is 					substrate-binding region	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_24_3278_s_110	11751633	( E) Emi1 binds the substrate-binding region (SBR) of Cdc20.	bind
3028	1	2068	6	10	NULL	0	NULL	Nup98-Hoxa9 	GP		bind					Hoxa9 	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_embo_25_7_1469_s_119	16525506	( E) EMSA. Smad4 dose-dependently inhibits the DNA-binding ability of Nup98-Hoxa9 to   Hoxa9 promoter probe, whether in the absence or in the presence of PBX1a, at molar ratios  of 0.2, 0.4 and 1 of Smad4 compared to Nup98-Hoxa9.	bind
3029	2	2068	6	10	NULL	0	NULL	Smad4	GP		inhibits		dose dependently			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_7_1469_s_119	16525506	( E) EMSA. Smad4 dose-dependently inhibits the DNA-binding ability of Nup98-Hoxa9 to   Hoxa9 promoter probe, whether in the absence or in the presence of PBX1a, at molar ratios  of 0.2, 0.4 and 1 of Smad4 compared to Nup98-Hoxa9.	bind
4701	1	2068	7	10	NULL	0	NULL	Nup98-Hoxa9	GP		binds					Hoxa9	GP			promoter 	NULL		NULL	NULL	NULL	NULL	gw70_embo_25_7_1469_s_119	16525506	( E) EMSA. Smad4 dose-dependently inhibits the DNA-binding ability of Nup98-Hoxa9 to   Hoxa9 promoter probe, whether in the absence or in the presence of PBX1a, at molar ratios  of 0.2, 0.4 and 1 of Smad4 compared to Nup98-Hoxa9.	bind
4702	2	2068	7	10	NULL	0	NULL	Smad4	GP		inhibits		dose-dependently			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_7_1469_s_119	16525506	( E) EMSA. Smad4 dose-dependently inhibits the DNA-binding ability of Nup98-Hoxa9 to   Hoxa9 promoter probe, whether in the absence or in the presence of PBX1a, at molar ratios  of 0.2, 0.4 and 1 of Smad4 compared to Nup98-Hoxa9.	bind
3030	1	2069	6	10	NULL	0	NULL	GATA-1	GP		bind					EKLF	GP			enhancer	NULL		NULL	NULL	NULL	NULL	gw70_embo_25_14_3264_s_260	16858405	( E) GATA-1 binding to the EKLF enhancer is increased when MAPK signalling is inhibited.	bind
3031	2	2069	6	10	NULL	0	NULL	MAPK signalling	Process	inhibition of	increases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_14_3264_s_260	16858405	( E) GATA-1 binding to the EKLF enhancer is increased when MAPK signalling is inhibited.	bind
4708	1	2069	7	10	NULL	0	NULL	GATA-1	GP		binds					EKLF 	GP			enhancer	NULL		NULL	NULL	NULL	NULL	gw70_embo_25_14_3264_s_260	16858405	( E) GATA-1 binding to the EKLF enhancer is increased when MAPK signalling is inhibited.	bind
4710	2	2069	7	10	NULL	0	NULL	MAPK signalling	Process	inhibition of	increases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_14_3264_s_260	16858405	( E) GATA-1 binding to the EKLF enhancer is increased when MAPK signalling is inhibited.	bind
3032	1	2070	6	10	NULL	0	NULL	Ggamma5	GP		interacts		directly			AEBP1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_14_4004_s_142	10406805	( E) Ggamma5 directly interacts with AEBP1 and prevents binding of AEBP1 to AE-1 oligonucleotides.	bind
3033	2	2070	6	10	NULL	0	NULL	AEBP1	GP		bind					AE-1 oligonucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_14_4004_s_142	10406805	( E) Ggamma5 directly interacts with AEBP1 and prevents binding of AEBP1 to AE-1 oligonucleotides.	bind
3034	3	2070	6	10	NULL	0	NULL	statement 1	Process		prevents					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_14_4004_s_142	10406805	( E) Ggamma5 directly interacts with AEBP1 and prevents binding of AEBP1 to AE-1 oligonucleotides.	bind
4713	1	2070	7	10	NULL	0	NULL	Ggamma5	GP		interacts with		directly			AEBP1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_14_4004_s_142	10406805	( E) Ggamma5 directly interacts with AEBP1 and prevents binding of AEBP1 to AE-1 oligonucleotides.	bind
4714	2	2070	7	10	NULL	0	NULL	AEBP1	GP		binds					AE-1 oligonucleotides	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_14_4004_s_142	10406805	( E) Ggamma5 directly interacts with AEBP1 and prevents binding of AEBP1 to AE-1 oligonucleotides.	bind
4715	3	2070	7	10	NULL	0	NULL	statement 1	Process		prevents					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_14_4004_s_142	10406805	( E) Ggamma5 directly interacts with AEBP1 and prevents binding of AEBP1 to AE-1 oligonucleotides.	bind
3035	1	2072	6	10	NULL	0	NULL	NE	GP		bind					QseC	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_27_10420_s_71	16803956	( E) Graphical representation of the amount of [3]NE bound to QseC after incubation with 5 and 10 muM [3]NE alone or in the presence of 50 muM PE.	bind
4716	1	2072	7	10	NULL	0	NULL	NE	GP		binds					QseC	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_27_10420_s_71	16803956	( E) Graphical representation of the amount of [3]NE bound to QseC after incubation with 5 and 10 muM [3]NE alone or in the presence of 50 muM PE.	bind
3036	1	2073	6	10	NULL	0	NULL	GroEL	GP		bind					Gbeta	GP		WD40 repeats		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_22_8360_s_96	16717193	( E) GroEL binding to individual WD40 repeats of Gbeta.	bind
4719	1	2073	7	10	NULL	0	NULL	GroEL	GP		binds					Gbeta	GP		WD40 repeats		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_22_8360_s_96	16717193	( E) GroEL binding to individual WD40 repeats of Gbeta.	bind
3037	1	2074	6	10	NULL	0	NULL	Smad3	GP		bind					CBP	GP				NULL	293T cells	NULL	NULL	NULL	NULL	gw70_embo_24_14_2543_s_136	15990875	( E) HDAC5 decreases the binding of Smad3 to CBP. 293T cells expressing the indicated  proteins were subject to immunoprecipitation with anti-Flag antibodies.	bind
3038	2	2074	6	10	NULL	0	NULL	HDAC5	GP		decreases					statement 1	Process				NULL	293T cells	NULL	NULL	NULL	NULL	gw70_embo_24_14_2543_s_136	15990875	( E) HDAC5 decreases the binding of Smad3 to CBP. 293T cells expressing the indicated  proteins were subject to immunoprecipitation with anti-Flag antibodies.	bind
4720	1	2074	7	10	NULL	0	NULL	Smad3	GP		binds					CBP	GP				NULL	293T cells	NULL	NULL	NULL	NULL	gw70_embo_24_14_2543_s_136	15990875	( E) HDAC5 decreases the binding of Smad3 to CBP. 293T cells expressing the indicated  proteins were subject to immunoprecipitation with anti-Flag antibodies.	bind
4721	2	2074	7	10	NULL	0	NULL	HDAC5	GP		decreases					statement 1	Process				NULL	293T cells	NULL	NULL	NULL	NULL	gw70_embo_24_14_2543_s_136	15990875	( E) HDAC5 decreases the binding of Smad3 to CBP. 293T cells expressing the indicated  proteins were subject to immunoprecipitation with anti-Flag antibodies.	bind
3039	1	2075	6	10	NULL	0	NULL	ice1	GP	mutant	bind					MYC-2 DNA fragment	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_8_1043_s_170	12672693	( E) ice1 mutant protein also binds to the MYC-2 DNA fragment.	bind
4722	1	2075	7	10	NULL	0	NULL	ice1	GP	mutant	binds					MYC-2 DNA fragment	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_8_1043_s_170	12672693	( E) ice1 mutant protein also binds to the MYC-2 DNA fragment.	bind
3084	1	2076	6	10	NULL	0	NULL	IgG	GP		bind					B3 protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_115_5_1352_s_52	15841210	( E) IEF immunoblot with CSF (C) and serum (S) from 3 MS patients (adjusted to 10 mg  IgG/l) was performed to compare IgG binding patterns to proteins B3, C5, and G4.	bind
3085	2	2076	6	10	NULL	0	NULL	IgG	GP		bind					C5 protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_115_5_1352_s_52	15841210	( E) IEF immunoblot with CSF (C) and serum (S) from 3 MS patients (adjusted to 10 mg  IgG/l) was performed to compare IgG binding patterns to proteins B3, C5, and G4.	bind
3086	3	2076	6	10	NULL	0	NULL	IgG	GP		bind					G4 protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_115_5_1352_s_52	15841210	( E) IEF immunoblot with CSF (C) and serum (S) from 3 MS patients (adjusted to 10 mg  IgG/l) was performed to compare IgG binding patterns to proteins B3, C5, and G4.	bind
4723	1	2076	7	10	NULL	0	NULL	IgG	GP		binds					B3 proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_115_5_1352_s_52	15841210	( E) IEF immunoblot with CSF (C) and serum (S) from 3 MS patients (adjusted to 10 mg  IgG/l) was performed to compare IgG binding patterns to proteins B3, C5, and G4.	bind
4724	2	2076	7	10	NULL	0	NULL	IgG	GP		binds					C5 proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_115_5_1352_s_52	15841210	( E) IEF immunoblot with CSF (C) and serum (S) from 3 MS patients (adjusted to 10 mg  IgG/l) was performed to compare IgG binding patterns to proteins B3, C5, and G4.	bind
4725	3	2076	7	10	NULL	0	NULL	IgG	GP		binds					G4 proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_115_5_1352_s_52	15841210	( E) IEF immunoblot with CSF (C) and serum (S) from 3 MS patients (adjusted to 10 mg  IgG/l) was performed to compare IgG binding patterns to proteins B3, C5, and G4.	bind
3087	1	2077	6	10	NULL	0	NULL	IgG1	GP		bind					MDA-LDL 	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_3_427_s_169	15286809	( E) IgG1 binding to MDA-LDL ( F), IgM binding to OxLDL, and ( G) T15/EO6 antibodies of individual plasmas at 1:250 dilution before and after immunization.	bind
3088	2	2077	6	10	NULL	0	NULL	IgM	GP		bind					OxLDL	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_3_427_s_169	15286809	( E) IgG1 binding to MDA-LDL ( F), IgM binding to OxLDL, and ( G) T15/EO6 antibodies of individual plasmas at 1:250 dilution before and after immunization.	bind
3089	3	2077	6	10	NULL	0	NULL	IgM	GP		bind					T15/EO6 antibodies	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_3_427_s_169	15286809	( E) IgG1 binding to MDA-LDL ( F), IgM binding to OxLDL, and ( G) T15/EO6 antibodies of individual plasmas at 1:250 dilution before and after immunization.	bind
4726	1	2077	7	10	NULL	0	NULL	IgG1	GP		binds to					 MDA-LDL	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_3_427_s_169	15286809	( E) IgG1 binding to MDA-LDL ( F), IgM binding to OxLDL, and ( G) T15/EO6 antibodies of individual plasmas at 1:250 dilution before and after immunization.	bind
4727	2	2077	7	10	NULL	0	NULL	IgM	GP		binds					OxLDL	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_3_427_s_169	15286809	( E) IgG1 binding to MDA-LDL ( F), IgM binding to OxLDL, and ( G) T15/EO6 antibodies of individual plasmas at 1:250 dilution before and after immunization.	bind
46282	3	2077	7	10	NULL	0	NULL	IgM	GP		bind					T15/EO6 antibodies	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_3_427_s_169	15286809	( E) IgG1 binding to MDA-LDL ( F), IgM binding to OxLDL, and ( G) T15/EO6 antibodies of individual plasmas at 1:250 dilution before and after immunization.	bind
3090	1	2078	6	10	NULL	0	NULL	p53	GP		bind					CHC	GP				NULL	H1299 cells	NULL	NULL	NULL	NULL	gw70_genesdev_20_9_1087_s_188	16618797	( E) Inhibition of the association of p53 with CHC by CLCb in H1299 cells through direct  binding of CLCb to CHC.	bind
3091	2	2078	6	10	NULL	0	NULL	CLCb	GP		bind		directly			CHC	GP				NULL	H1299 cells	NULL	NULL	NULL	NULL	gw70_genesdev_20_9_1087_s_188	16618797	( E) Inhibition of the association of p53 with CHC by CLCb in H1299 cells through direct  binding of CLCb to CHC.	bind
3092	3	2078	6	10	NULL	0	NULL	statement 2	Process		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_20_9_1087_s_188	16618797	( E) Inhibition of the association of p53 with CHC by CLCb in H1299 cells through direct  binding of CLCb to CHC.	bind
4728	1	2078	7	10	NULL	0	NULL	p53	GP		binds					CHC	GP				NULL	H1299 cells	NULL	NULL	NULL	NULL	gw70_genesdev_20_9_1087_s_188	16618797	( E) Inhibition of the association of p53 with CHC by CLCb in H1299 cells through direct  binding of CLCb to CHC.	bind
4729	2	2078	7	10	NULL	0	NULL	CLCb	GP		binds		directly			CHC	GP				NULL	H1299 cells	NULL	NULL	NULL	NULL	gw70_genesdev_20_9_1087_s_188	16618797	( E) Inhibition of the association of p53 with CHC by CLCb in H1299 cells through direct  binding of CLCb to CHC.	bind
4730	3	2078	7	10	NULL	0	NULL	statement 2	Process		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_20_9_1087_s_188	16618797	( E) Inhibition of the association of p53 with CHC by CLCb in H1299 cells through direct  binding of CLCb to CHC.	bind
3093	1	2079	6	10	NULL	0	NULL	KLF4	GP		bind		directly			Cx26	GP	proximal		promoter	NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_5_1243_s_87	16628254	( E) KLF4 binds directly to the proximal Cx26 promoter.	bind
4731	1	2079	7	10	NULL	0	NULL	KLF4	GP		binds		directly			Cx26	GP	proximal		promoter	NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_5_1243_s_87	16628254	( E) KLF4 binds directly to the proximal Cx26 promoter.	bind
3094	1	2080	6	10	NULL	0	NULL	VP16-ERalpha	GP	wild type	bind					peptides	AminoAcid	GAL4-DBD-tagged;;wild type			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_10_3593_s_168	15728727	( E) Mammalian two-hybrid receptor binding assay of GAL4-DBD-tagged wild type and mutant  peptides to VP16-ERalpha wild type.	bind
3095	2	2080	6	10	NULL	0	NULL	VP16-ERalpha	GP	wild type	bind					peptides	AminoAcid	GAL4-DBD-tagged;;mutant type			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_10_3593_s_168	15728727	( E) Mammalian two-hybrid receptor binding assay of GAL4-DBD-tagged wild type and mutant  peptides to VP16-ERalpha wild type.	bind
4732	1	2080	7	10	NULL	0	NULL	peptide	AminoAcid	wild type;;GAL4-DBD-tagged	bind					VP16-ERalpha 	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_10_3593_s_168	15728727	( E) Mammalian two-hybrid receptor binding assay of GAL4-DBD-tagged wild type and mutant  peptides to VP16-ERalpha wild type.	bind
4733	2	2080	7	10	NULL	0	NULL	peptide	AminoAcid	mutant;;GAL4-DBD-tagged 	bind					VP16-ERalpha	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_10_3593_s_168	15728727	( E) Mammalian two-hybrid receptor binding assay of GAL4-DBD-tagged wild type and mutant  peptides to VP16-ERalpha wild type.	bind
3096	1	2081	6	10	NULL	0	NULL	Mant-GTP	Chemical		bind					RacC	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_7_1620_s_184	11285226	( E) Mant-GTP binding to RacC or ( F) mant-GDP dissociation from RacE in the presence or absence of 8 muM 2D.	bind
3097	2	2081	6	10	NULL	0	NULL	Mant-GDP	Chemical		dissociates from					RacE	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_7_1620_s_184	11285226	( E) Mant-GTP binding to RacC or ( F) mant-GDP dissociation from RacE in the presence or absence of 8 muM 2D.	bind
4734	1	2081	7	10	NULL	0	NULL	Mant-GTP	Chemical		binds					RacC	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_7_1620_s_184	11285226	( E) Mant-GTP binding to RacC or ( F) mant-GDP dissociation from RacE in the presence or absence of 8 muM 2D.	bind
4735	2	2081	7	10	NULL	0	NULL	mant-GDP 	Chemical		dissociates from					RacE	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_7_1620_s_184	11285226	( E) Mant-GTP binding to RacC or ( F) mant-GDP dissociation from RacE in the presence or absence of 8 muM 2D.	bind
3098	1	2082	6	10	NULL	0	NULL	Nurr1	GP		bind					DAT	GP			promoter sequences	NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_8_2874_s_108	16477036	( E) Nurr1 and Pitx3 bind cooperatively to DAT promoter sequences.	bind
3099	2	2082	6	10	NULL	0	NULL	Pitx3	GP		bind					DAT	GP			promoter sequences	NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_8_2874_s_108	16477036	( E) Nurr1 and Pitx3 bind cooperatively to DAT promoter sequences.	bind
3100	3	2082	6	10	NULL	0	NULL	statement 1	Process		cooperates with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_8_2874_s_108	16477036	( E) Nurr1 and Pitx3 bind cooperatively to DAT promoter sequences.	bind
4736	1	2082	7	10	NULL	0	NULL	Nurr1	GP		binds					DAT	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_8_2874_s_108	16477036	( E) Nurr1 and Pitx3 bind cooperatively to DAT promoter sequences.	bind
4737	2	2082	7	10	NULL	0	NULL	Pitx3	GP		bind					DAT	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_8_2874_s_108	16477036	( E) Nurr1 and Pitx3 bind cooperatively to DAT promoter sequences.	bind
4738	3	2082	7	10	NULL	0	NULL	statement 1	Process		occurs in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_8_2874_s_108	16477036	( E) Nurr1 and Pitx3 bind cooperatively to DAT promoter sequences.	bind
3101	1	2083	6	10	NULL	0	NULL	FOXO1	GP		bind					InR 	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_20_2435_s_227	16230533	( E) Phosphorylation by Akt prevents binding of FOXO1 to the InR promoter probe.	bind
3102	2	2083	6	10	NULL	0	NULL	Akt	GP		phosphorylate					FOXO1	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_20_2435_s_227	16230533	( E) Phosphorylation by Akt prevents binding of FOXO1 to the InR promoter probe.	bind
4029	3	2083	6	10	NULL	0	NULL	statement 2	Process		prevents					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_20_2435_s_227	16230533	( E) Phosphorylation by Akt prevents binding of FOXO1 to the InR promoter probe.	bind
4739	1	2083	7	10	NULL	0	NULL	FOXO1	GP		binds					 InR 	GP			promoter 	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_20_2435_s_227	16230533	( E) Phosphorylation by Akt prevents binding of FOXO1 to the InR promoter probe.	bind
4740	2	2083	7	10	NULL	0	NULL	Akt	GP		phosphorylates					FOXO1	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_20_2435_s_227	16230533	( E) Phosphorylation by Akt prevents binding of FOXO1 to the InR promoter probe.	bind
4741	3	2083	7	10	NULL	0	NULL	statement 2	Process		prevents					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_20_2435_s_227	16230533	( E) Phosphorylation by Akt prevents binding of FOXO1 to the InR promoter probe.	bind
3103	1	2084	6	10	NULL	0	NULL	Pin-1	GP		bind					cyclin D1	GP	phosphorylated	Thr-286		NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_3_1335_s_170	11805292	( E) Pin1 binds cyclin D1 phosphorylated on Thr-286.	bind
4742	1	2084	7	10	NULL	0	NULL	Pin1	GP		binds					cyclin D1	GP	phosphorylated	 Thr-286 		NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_3_1335_s_170	11805292	( E) Pin1 binds cyclin D1 phosphorylated on Thr-286.	bind
3105	1	2085	6	10	NULL	0	NULL	Pmo25	GP		bind					Nak1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_embo_24_17_3012_s_102	16096637	( E) Pmo25 binds to Nak1  in vitro.	bind
4743	1	2085	7	10	NULL	0	NULL	Pmo25	GP		binds					Nak1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_embo_24_17_3012_s_102	16096637	( E) Pmo25 binds to Nak1  in vitro.	bind
3107	1	2086	6	10	NULL	0	NULL	120 kD protein	GP	purified	bind					SRE-containing probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_19_2482_s_78	9334314	( E) Purifed 120 kD protein binds to an SRE-containing probe.	bind
4744	1	2086	7	10	NULL	0	NULL	120 kD protein	GP	purified	binds to					SRE-containing probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_19_2482_s_78	9334314	( E) Purifed 120 kD protein binds to an SRE-containing probe.	bind
3108	1	2087	6	10	NULL	0	NULL	p53	GP		bind					p21	GP			promoter	NULL	IMR90 	NULL	NULL	NULL	NULL	gw70_genesdev_19_2_196_s_126	15655109	( E) Quantitative analysis of p53 binding to the  p21 promoter in control IMR90 and IMR90 depleted of p400.	bind
3109	2	2087	6	10	NULL	0	NULL	p53	GP		bind					p21	GP			promoter	NULL	IMR90 depleted of p400	NULL	NULL	NULL	NULL	gw70_genesdev_19_2_196_s_126	15655109	( E) Quantitative analysis of p53 binding to the  p21 promoter in control IMR90 and IMR90 depleted of p400.	bind
4745	1	2087	7	10	NULL	0	NULL	p53	GP		binds to					 p21	GP			promoter	NULL	in IMR90	NULL	NULL	NULL	NULL	gw70_genesdev_19_2_196_s_126	15655109	( E) Quantitative analysis of p53 binding to the  p21 promoter in control IMR90 and IMR90 depleted of p400.	bind
4746	2	2087	7	10	NULL	0	NULL	p53	GP		binds					p21	GP			promoter	NULL	in IMR90 depleted of p400	NULL	NULL	NULL	NULL	gw70_genesdev_19_2_196_s_126	15655109	( E) Quantitative analysis of p53 binding to the  p21 promoter in control IMR90 and IMR90 depleted of p400.	bind
3111	1	2088	6	10	NULL	0	NULL	GATA-1	GP		bind					GATA-1	GP			HS1	NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_103	14715908	( E) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to  GATA- 1 HS1, alpha-globin HS-26, and  ALAS- 2 intron 8 in untreated and tamoxifen-treated (1 muM, 24 h) FOG-1 - / -  and FOG-1 - / - -ER - GATA-1 cells (mean  plus-or-minus  SEM of three independent experiments).	bind
3186	2	2088	6	10	NULL	0	NULL	GATA-1	GP		bind					alpha-globin	GP			HS-26	NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_103	14715908	( E) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to  GATA- 1 HS1, alpha-globin HS-26, and  ALAS- 2 intron 8 in untreated and tamoxifen-treated (1 muM, 24 h) FOG-1 - / -  and FOG-1 - / - -ER - GATA-1 cells (mean  plus-or-minus  SEM of three independent experiments).	bind
3187	3	2088	6	10	NULL	0	NULL	GATA-1	GP		bind					ALAS-2	GP			intron 8	NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_103	14715908	( E) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to  GATA- 1 HS1, alpha-globin HS-26, and  ALAS- 2 intron 8 in untreated and tamoxifen-treated (1 muM, 24 h) FOG-1 - / -  and FOG-1 - / - -ER - GATA-1 cells (mean  plus-or-minus  SEM of three independent experiments).	bind
3188	4	2088	6	10	NULL	0	NULL	GATA-2	GP		bind					GATA-1	GP			HS1	NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_103	14715908	( E) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to  GATA- 1 HS1, alpha-globin HS-26, and  ALAS- 2 intron 8 in untreated and tamoxifen-treated (1 muM, 24 h) FOG-1 - / -  and FOG-1 - / - -ER - GATA-1 cells (mean  plus-or-minus  SEM of three independent experiments).	bind
3189	5	2088	6	10	NULL	0	NULL	GATA-2	GP		bind					alpha-globin	GP			HS-26	NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_103	14715908	( E) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to  GATA- 1 HS1, alpha-globin HS-26, and  ALAS- 2 intron 8 in untreated and tamoxifen-treated (1 muM, 24 h) FOG-1 - / -  and FOG-1 - / - -ER - GATA-1 cells (mean  plus-or-minus  SEM of three independent experiments).	bind
3190	6	2088	6	10	NULL	0	NULL	GATA-2	GP		bind					ALAS-2	GP			intron 8	NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_103	14715908	( E) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to  GATA- 1 HS1, alpha-globin HS-26, and  ALAS- 2 intron 8 in untreated and tamoxifen-treated (1 muM, 24 h) FOG-1 - / -  and FOG-1 - / - -ER - GATA-1 cells (mean  plus-or-minus  SEM of three independent experiments).	bind
4747	1	2088	7	10	NULL	0	NULL	GATA-1	GP		binds					GATA- 1 	GP			HS1	NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_103	14715908	( E) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to  GATA- 1 HS1, alpha-globin HS-26, and  ALAS- 2 intron 8 in untreated and tamoxifen-treated (1 muM, 24 h) FOG-1 - / -  and FOG-1 - / - -ER - GATA-1 cells (mean  plus-or-minus  SEM of three independent experiments).	bind
4748	2	2088	7	10	NULL	0	NULL	GATA-1	GP		binds					alpha-globin 	GP			HS-26	NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_103	14715908	( E) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to  GATA- 1 HS1, alpha-globin HS-26, and  ALAS- 2 intron 8 in untreated and tamoxifen-treated (1 muM, 24 h) FOG-1 - / -  and FOG-1 - / - -ER - GATA-1 cells (mean  plus-or-minus  SEM of three independent experiments).	bind
4749	3	2088	7	10	NULL	0	NULL	GATA-1	GP		binds					ALAS- 2 	GP			intron 8	NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_103	14715908	( E) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to  GATA- 1 HS1, alpha-globin HS-26, and  ALAS- 2 intron 8 in untreated and tamoxifen-treated (1 muM, 24 h) FOG-1 - / -  and FOG-1 - / - -ER - GATA-1 cells (mean  plus-or-minus  SEM of three independent experiments).	bind
4750	4	2088	7	10	NULL	0	NULL	GATA-2	GP		binds					GATA- 1 	GP			HS1	NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_103	14715908	( E) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to  GATA- 1 HS1, alpha-globin HS-26, and  ALAS- 2 intron 8 in untreated and tamoxifen-treated (1 muM, 24 h) FOG-1 - / -  and FOG-1 - / - -ER - GATA-1 cells (mean  plus-or-minus  SEM of three independent experiments).	bind
4751	5	2088	7	10	NULL	0	NULL	GATA-2	GP		binds					alpha-globin 	GP			HS-26	NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_103	14715908	( E) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to  GATA- 1 HS1, alpha-globin HS-26, and  ALAS- 2 intron 8 in untreated and tamoxifen-treated (1 muM, 24 h) FOG-1 - / -  and FOG-1 - / - -ER - GATA-1 cells (mean  plus-or-minus  SEM of three independent experiments).	bind
4752	6	2088	7	10	NULL	0	NULL	GATA-2 	GP		binds					ALAS- 2 	GP			intron 8	NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_4_980_s_103	14715908	( E) Quantitative ChIP analysis of GATA-1 and GATA-2 binding to  GATA- 1 HS1, alpha-globin HS-26, and  ALAS- 2 intron 8 in untreated and tamoxifen-treated (1 muM, 24 h) FOG-1 - / -  and FOG-1 - / - -ER - GATA-1 cells (mean  plus-or-minus  SEM of three independent experiments).	bind
3113	1	2089	6	10	NULL	0	NULL	palmitate	Chemical		bind					paralemmin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_143_3_795_s_249	9813098	( E) Release of paralemmin-bound [3]palmitate by hydrolysis with hydroxylamine.	bind
46183	2	2089	6	10	NULL	0	NULL	statement 1	GP		is hydrolysed with					hydroxylamine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_143_3_795_s_249	9813098	( E) Release of paralemmin-bound [3]palmitate by hydrolysis with hydroxylamine.	bind
46184	3	2089	6	10	NULL	0	NULL	statement 2	Process		release					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_143_3_795_s_249	9813098	( E) Release of paralemmin-bound [3]palmitate by hydrolysis with hydroxylamine.	bind
4759	1	2089	7	10	NULL	0	NULL	paralemmin	GP		binds					palmitate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_143_3_795_s_249	9813098	( E) Release of paralemmin-bound [3]palmitate by hydrolysis with hydroxylamine.	bind
4760	2	2089	7	10	NULL	0	NULL	statement 1	GP		is hydrolysed with					hydroxylamine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_143_3_795_s_249	9813098	( E) Release of paralemmin-bound [3]palmitate by hydrolysis with hydroxylamine.	bind
4761	3	2089	7	10	NULL	0	NULL	statement 2	Process		release					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_143_3_795_s_249	9813098	( E) Release of paralemmin-bound [3]palmitate by hydrolysis with hydroxylamine.	bind
3115	1	2090	6	10	NULL	0	NULL	RNA Pol II	GP		bind					BNA1	GP			promoter	NULL	in vivo in wild type cells 	NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_155	15861138	( E) RNA Pol II binding to  BNA1 and  URA1 promoters  in vivo was determined by ChIP using chromatin from wild-type (WT) or  mot1-42 mutant cells.	bind
3116	2	2090	6	10	NULL	0	NULL	RNA Pol II	GP		bind					URA1	GP			promoter	NULL	in vivo in wild type cells	NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_155	15861138	( E) RNA Pol II binding to  BNA1 and  URA1 promoters  in vivo was determined by ChIP using chromatin from wild-type (WT) or  mot1-42 mutant cells.	bind
3119	3	2090	6	10	NULL	0	NULL	RNA Pol II	GP		bind					BNA1	GP			promoter	NULL	in vivo in mot1-42 mutant cells	NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_155	15861138	( E) RNA Pol II binding to  BNA1 and  URA1 promoters  in vivo was determined by ChIP using chromatin from wild-type (WT) or  mot1-42 mutant cells.	bind
3120	4	2090	6	10	NULL	0	NULL	RNA Pol II	GP		bind					URA1	GP			promoter	NULL	in vivo in mot1-42 mutant cells	NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_155	15861138	( E) RNA Pol II binding to  BNA1 and  URA1 promoters  in vivo was determined by ChIP using chromatin from wild-type (WT) or  mot1-42 mutant cells.	bind
4762	1	2090	7	10	NULL	0	NULL	RNA Pol II	GP		binds to					BNA1	GP			promoter	NULL	in vivo from wild-type (WT) cells	NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_155	15861138	( E) RNA Pol II binding to  BNA1 and  URA1 promoters  in vivo was determined by ChIP using chromatin from wild-type (WT) or  mot1-42 mutant cells.	bind
4763	2	2090	7	10	NULL	0	NULL	RNA Pol II	GP		binds to					URA1	GP			promoter	NULL	in vivo from wild-type (WT) cells	NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_155	15861138	( E) RNA Pol II binding to  BNA1 and  URA1 promoters  in vivo was determined by ChIP using chromatin from wild-type (WT) or  mot1-42 mutant cells.	bind
4764	3	2090	7	10	NULL	0	NULL	RNA Pol II	GP		binds to					BNA1	GP			promoter	NULL	in vivo from mot1-42 mutant cells	NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_155	15861138	( E) RNA Pol II binding to  BNA1 and  URA1 promoters  in vivo was determined by ChIP using chromatin from wild-type (WT) or  mot1-42 mutant cells.	bind
4765	4	2090	7	10	NULL	0	NULL	RNA Pol II	GP		binds to					URA1	GP			promoter	NULL	in vivo from mot1-42 mutant cells	NULL	NULL	NULL	NULL	gw70_embo_24_9_1717_s_155	15861138	( E) RNA Pol II binding to  BNA1 and  URA1 promoters  in vivo was determined by ChIP using chromatin from wild-type (WT) or  mot1-42 mutant cells.	bind
3121	1	2091	6	10	NULL	0	NULL	myostatin	GP		bind					ActRIIB	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_16_9306_s_65	11459935	( e) Scatchard analysis of the data shown in  d. ( f) Inhibition of myostatin binding to ActRIIB by follistatin (diamonds) and the propeptide (circles).	bind
3123	2	2091	6	10	NULL	0	NULL	follistatin	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_16_9306_s_65	11459935	( e) Scatchard analysis of the data shown in  d. ( f) Inhibition of myostatin binding to ActRIIB by follistatin (diamonds) and the propeptide (circles).	bind
3124	3	2091	6	10	NULL	0	NULL	propeptide	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_16_9306_s_65	11459935	( e) Scatchard analysis of the data shown in  d. ( f) Inhibition of myostatin binding to ActRIIB by follistatin (diamonds) and the propeptide (circles).	bind
4766	1	2091	7	10	NULL	0	NULL	myostatin	GP		binds to					ActRIIB	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_16_9306_s_65	11459935	( e) Scatchard analysis of the data shown in  d. ( f) Inhibition of myostatin binding to ActRIIB by follistatin (diamonds) and the propeptide (circles).	bind
4767	2	2091	7	10	NULL	0	NULL	follistatin	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_16_9306_s_65	11459935	( e) Scatchard analysis of the data shown in  d. ( f) Inhibition of myostatin binding to ActRIIB by follistatin (diamonds) and the propeptide (circles).	bind
4768	3	2091	7	10	NULL	0	NULL	propeptide	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_16_9306_s_65	11459935	( e) Scatchard analysis of the data shown in  d. ( f) Inhibition of myostatin binding to ActRIIB by follistatin (diamonds) and the propeptide (circles).	bind
3127	1	2092	6	10	NULL	0	NULL	calcineurin A	GP	residues	bind					atrogin-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_8_1058_s_89	15489953	( E) Schematic representations of calcineurin A residues that bind to atrogin-1.	bind
4769	1	2092	7	10	NULL	0	NULL	calcineurin A	GP	residues of	binds					atrogin-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_8_1058_s_89	15489953	( E) Schematic representations of calcineurin A residues that bind to atrogin-1.	bind
3130	1	2093	6	10	NULL	0	NULL	ERalpha	GP		bind					Rsk2	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_13_3484_s_109	11432835	( E) Schematic showing homology between the region in ERalpha that binds to Rsk2 and the analogous region of ERbeta.	bind
46185	2	2093	6	10	NULL	0	NULL	ERalpha	GP	binding region of	is homologous to					ERbeta	GP	binding region of 			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_13_3484_s_109	11432835	( E) Schematic showing homology between the region in ERalpha that binds to Rsk2 and the analogous region of ERbeta.	bind
4770	1	2093	7	10	NULL	0	NULL	ERalpha	GP		binds to					Rsk2	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_13_3484_s_109	11432835	( E) Schematic showing homology between the region in ERalpha that binds to Rsk2 and the analogous region of ERbeta.	bind
4771	2	2093	7	10	NULL	0	NULL	 ERalpha	GP	binding region	is homologous to					ERbeta	GP	binding region			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_13_3484_s_109	11432835	( E) Schematic showing homology between the region in ERalpha that binds to Rsk2 and the analogous region of ERbeta.	bind
3133	1	2095	6	10	NULL	0	NULL	Smads	GP		bind					Xtwn	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_15_8358_s_138	10890911	( E) Smads and LEF1 expressed in mammalian cells bind to the Xtwn promoter.	bind
3134	2	2095	6	10	NULL	0	NULL	LEF1	GP		bind					Xtwn	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_15_8358_s_138	10890911	( E) Smads and LEF1 expressed in mammalian cells bind to the Xtwn promoter.	bind
46186	3	2095	6	10	NULL	0	NULL	Smads	GP		is expressed in					mammalian cell	Cell				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_15_8358_s_138	10890911	( E) Smads and LEF1 expressed in mammalian cells bind to the Xtwn promoter.	bind
46187	4	2095	6	10	NULL	0	NULL	LEF1	GP		is expressed in					mammalian cell	Cell				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_15_8358_s_138	10890911	( E) Smads and LEF1 expressed in mammalian cells bind to the Xtwn promoter.	bind
4772	1	2095	7	10	NULL	0	NULL	Smads 	GP		bind					Xtwn	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_15_8358_s_138	10890911	( E) Smads and LEF1 expressed in mammalian cells bind to the Xtwn promoter.	bind
4773	2	2095	7	10	NULL	0	NULL	LEF1	GP		bind					Xtwn	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_15_8358_s_138	10890911	( E) Smads and LEF1 expressed in mammalian cells bind to the Xtwn promoter.	bind
4774	3	2095	7	10	NULL	0	NULL	Smads	GP		expressed in					mammalian cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_15_8358_s_138	10890911	( E) Smads and LEF1 expressed in mammalian cells bind to the Xtwn promoter.	bind
4775	4	2095	7	10	NULL	0	NULL	LEF1	GP		expressed in					mammalian cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_15_8358_s_138	10890911	( E) Smads and LEF1 expressed in mammalian cells bind to the Xtwn promoter.	bind
3135	1	2096	6	10	NULL	0	NULL	Sf-H2	GP	recombinant;;iodinated	bind		species specific			bindin particles	GP	purified			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_20_2502_s_62	14561772	( E) Species-specific binding of recombinant iodinated  Sf-H2 to purified bindin particles.	bind
4776	1	2096	7	10	NULL	0	NULL	Sf-H2	GP	recombinant;;iodinated	binds		species specific			bindin particles	GP	purified			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_20_2502_s_62	14561772	( E) Species-specific binding of recombinant iodinated  Sf-H2 to purified bindin particles.	bind
3136	1	2097	6	10	NULL	0	NULL	kappaB-Ras	GP		bind		specifically			GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_287_5454_869_s_40	10657303	( E) Specific binding of kappaB-Ras to GTP.	bind
4778	1	2097	7	10	NULL	0	NULL	 kappaB-Ras	GP		binds		specifically			GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_287_5454_869_s_40	10657303	( E) Specific binding of kappaB-Ras to GTP.	bind
3141	2	2098	6	10	NULL	0	NULL	SRC1	GP		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_10_2083_s_124	15103326	( E) SRC1 binds to DNA-bound RXR, in a 9 -cis RA-dependent manner.	bind
3142	3	2098	6	10	NULL	0	NULL	statement 2	Process		is dependent on					9 -cis RA	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_10_2083_s_124	15103326	( E) SRC1 binds to DNA-bound RXR, in a 9 -cis RA-dependent manner.	bind
60879	1	2098	6	10	NULL	0	NULL	RXR	GP		bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_embo_23_10_2083_s_124	15103326	( E) SRC1 binds to DNA-bound RXR, in a 9 -cis RA-dependent manner.	bind
4779	2	2098	7	10	NULL	0	NULL	SRC1	GP		binds to					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_10_2083_s_124	15103326	( E) SRC1 binds to DNA-bound RXR, in a 9 -cis RA-dependent manner.	bind
4780	3	2098	7	10	NULL	0	NULL	statement 2	Process		is dependent on					9 -cis RA	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_10_2083_s_124	15103326	( E) SRC1 binds to DNA-bound RXR, in a 9 -cis RA-dependent manner.	bind
60880	1	2098	7	10	NULL	0	NULL	RXR	GP		bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_embo_23_10_2083_s_124	15103326	( E) SRC1 binds to DNA-bound RXR, in a 9 -cis RA-dependent manner.	bind
3143	1	2099	6	10	NULL	0	NULL	EAT-2	GP	mouse	bind					CD150 peptide	GP		pTyr281		NULL		NULL	NULL	NULL	NULL	gw60_embo_20_21_5840_s_59	11689425	( E) Superimposition of the mouse EAT-2 and human SH2D1A structures bound to the CD150 pTyr281 peptide.	bind
3144	2	2099	6	10	NULL	0	NULL	SH2D1A	GP	human	bind					CD150 peptide	GP		pTyr281		NULL		NULL	NULL	NULL	NULL	gw60_embo_20_21_5840_s_59	11689425	( E) Superimposition of the mouse EAT-2 and human SH2D1A structures bound to the CD150 pTyr281 peptide.	bind
4783	1	2099	7	10	NULL	0	NULL	EAT-2	GP	mouse	binds to					CD150  peptide	GP		pTyr281		NULL		NULL	NULL	NULL	NULL	gw60_embo_20_21_5840_s_59	11689425	( E) Superimposition of the mouse EAT-2 and human SH2D1A structures bound to the CD150 pTyr281 peptide.	bind
4784	2	2099	7	10	NULL	0	NULL	SH2D1A	GP	human	binds to					CD150  peptide	GP		pTyr281		NULL		NULL	NULL	NULL	NULL	gw60_embo_20_21_5840_s_59	11689425	( E) Superimposition of the mouse EAT-2 and human SH2D1A structures bound to the CD150 pTyr281 peptide.	bind
3145	1	2101	6	10	NULL	0	NULL	p38	GP	mutant	bind					MNK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_466_s_291	11157753	( E) The binding of the mutant forms of p38 and ERK2 to MNK1.	bind
3146	2	2101	6	10	NULL	0	NULL	ERK2	GP	mutant	bind					MNK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_466_s_291	11157753	( E) The binding of the mutant forms of p38 and ERK2 to MNK1.	bind
4856	1	2101	7	10	NULL	0	NULL	p38 	GP	mutant	binds					MNK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_466_s_291	11157753	( E) The binding of the mutant forms of p38 and ERK2 to MNK1.	bind
4857	2	2101	7	10	NULL	0	NULL	ERK2	GP	Mutant	binds					MNK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_466_s_291	11157753	( E) The binding of the mutant forms of p38 and ERK2 to MNK1.	bind
3150	1	2102	6	10	NULL	0	NULL	axin	GP		bind					GSK-3beta	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_11_6371_s_121	10339594	( E) The coiled-coil RGS protein axin binds GSK-3beta, but does not interact with polycystin.	bind
3151	2	2102	6	10	NULL	0	NULL	axin	GP		does not bind					polycystin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_11_6371_s_121	10339594	( E) The coiled-coil RGS protein axin binds GSK-3beta, but does not interact with polycystin.	bind
45873	3	2102	6	10	NULL	0	NULL	axin	GP		is a type of					coiled-coil RGS protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_11_6371_s_121	10339594	( E) The coiled-coil RGS protein axin binds GSK-3beta, but does not interact with polycystin.	bind
4858	1	2102	7	10	NULL	0	NULL	axin	GP		binds					GSK-3beta	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_11_6371_s_121	10339594	( E) The coiled-coil RGS protein axin binds GSK-3beta, but does not interact with polycystin.	bind
4859	2	2102	7	10	NULL	0	NULL	axin	GP		does not bind					polycystin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_11_6371_s_121	10339594	( E) The coiled-coil RGS protein axin binds GSK-3beta, but does not interact with polycystin.	bind
45874	3	2102	7	10	NULL	0	NULL	axin	GP		is a type of					coiled-coil RGS protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_11_6371_s_121	10339594	( E) The coiled-coil RGS protein axin binds GSK-3beta, but does not interact with polycystin.	bind
3154	1	2103	6	10	NULL	0	NULL	mAb 196	GP		bind					Abeta	GP		N-terminus		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_21_7718_s_206	15894613	( E) The levels of salphaAPP released to the cells' media were analyzed after 24 and 48 h by Western blot  using mAb 196, which binds Abeta in the N terminus.	bind
4884	1	2103	7	10	NULL	0	NULL	mAb 196	GP		binds					Abeta	GP		N terminus		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_21_7718_s_206	15894613	( E) The levels of salphaAPP released to the cells' media were analyzed after 24 and 48 h by Western blot  using mAb 196, which binds Abeta in the N terminus.	bind
3156	1	2104	6	10	NULL	0	NULL	VEGF-C	GP		bind					VEGFR3	GP				NULL	corneal epithelium	NULL	NULL	NULL	NULL	gw70_pnas_103_30_11405_s_45	16849433	( E) VEGF-C binds to corneal epithelial VEGFR3 and leads to VEGFR3 activation.	bind
3158	2	2104	6	10	NULL	0	NULL	statement 1	Process		leads to					VEGFR3	GP	activation of			NULL	corneal epithelium	NULL	NULL	NULL	NULL	gw70_pnas_103_30_11405_s_45	16849433	( E) VEGF-C binds to corneal epithelial VEGFR3 and leads to VEGFR3 activation.	bind
4882	1	2104	7	10	NULL	0	NULL	VEGF-C 	GP		binds					VEGFR3	GP				NULL	corneal epithelium	NULL	NULL	NULL	NULL	gw70_pnas_103_30_11405_s_45	16849433	( E) VEGF-C binds to corneal epithelial VEGFR3 and leads to VEGFR3 activation.	bind
4883	2	2104	7	10	NULL	0	NULL	statement 1	Process		leads to					VEGFR3	GP	activation of			NULL	corneal epithelium	NULL	NULL	NULL	NULL	gw70_pnas_103_30_11405_s_45	16849433	( E) VEGF-C binds to corneal epithelial VEGFR3 and leads to VEGFR3 activation.	bind
3160	1	2105	6	10	NULL	0	NULL	ZO-3	GP		does not bind					ZO-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_1_199_s_151	9531559	( e) ZO-3  does not bind to ZO-2.	bind
4885	1	2105	7	10	NULL	0	NULL	ZO-3	GP		does not bind					ZO-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_1_199_s_151	9531559	( e) ZO-3  does not bind to ZO-2.	bind
3161	1	2106	6	10	NULL	0	NULL	synaptotagmin 2	GP	WT	bind					SNARE complexes	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_10_2039_s_66	16642042	( E, F) Binding of WT and I337N-mutant synaptotagmin 2 to SNARE complexes analyzed by immunoprecipitations.	bind
3162	2	2106	6	10	NULL	0	NULL	synaptotagmin 2	GP	mutant	bind			I337N		SNARE complexes	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_10_2039_s_66	16642042	( E, F) Binding of WT and I337N-mutant synaptotagmin 2 to SNARE complexes analyzed by immunoprecipitations.	bind
4887	1	2106	7	10	NULL	0	NULL	synaptotagmin 2	GP	WT	binds					SNARE complexes	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_10_2039_s_66	16642042	( E, F) Binding of WT and I337N-mutant synaptotagmin 2 to SNARE complexes analyzed by immunoprecipitations.	bind
4891	2	2106	7	10	NULL	0	NULL	synaptotagmin 2	GP	mutant	binds			I337N		SNARE complexes	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_10_2039_s_66	16642042	( E, F) Binding of WT and I337N-mutant synaptotagmin 2 to SNARE complexes analyzed by immunoprecipitations.	bind
3164	1	2107	6	10	NULL	0	NULL	TCF	GP		bind					nkd	GP			control region	NULL		NULL	NULL	NULL	NULL	gw70_embo_25_12_2735_s_163	16710294	( E, F) ChIP analysis shows overlapping binding of TCF (E) and CtBP (F) to the  nkd control region.	bind
3165	2	2107	6	10	NULL	0	NULL	CtBP	GP		bind					nkd	GP			control region	NULL		NULL	NULL	NULL	NULL	gw70_embo_25_12_2735_s_163	16710294	( E, F) ChIP analysis shows overlapping binding of TCF (E) and CtBP (F) to the  nkd control region.	bind
51551	3	2107	6	10	NULL	0	NULL	statement 1	Process		overlaps					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_12_2735_s_163	16710294	( E, F) ChIP analysis shows overlapping binding of TCF (E) and CtBP (F) to the  nkd control region.	bind
4894	1	2107	7	10	NULL	0	NULL	TCF	GP		binds					nkd	GP			control region	NULL		NULL	NULL	NULL	NULL	gw70_embo_25_12_2735_s_163	16710294	( E, F) ChIP analysis shows overlapping binding of TCF (E) and CtBP (F) to the  nkd control region.	bind
4896	2	2107	7	10	NULL	0	NULL	CtBP	GP		binds					nkd	GP			control region	NULL		NULL	NULL	NULL	NULL	gw70_embo_25_12_2735_s_163	16710294	( E, F) ChIP analysis shows overlapping binding of TCF (E) and CtBP (F) to the  nkd control region.	bind
4900	3	2107	7	10	NULL	0	NULL	statement 1	Process		overlaps					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_12_2735_s_163	16710294	( E, F) ChIP analysis shows overlapping binding of TCF (E) and CtBP (F) to the  nkd control region.	bind
3166	1	2108	6	10	NULL	0	NULL	PPARgamma/RXR	GP		bind					FXR 	GP			DR-1 element in promoter	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_18_2_157_s_108	14729567	( E,F) PPARgamma/RXR binds to the DR-1 elements in both FXR promoters.	bind
4898	1	2108	7	10	NULL	0	NULL	PPARgamma/RXR	GP		binds					FXR	GP			DR-1 elements in the promoter of	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_18_2_157_s_108	14729567	( E,F) PPARgamma/RXR binds to the DR-1 elements in both FXR promoters.	bind
3167	1	2109	6	10	NULL	0	NULL				bind			DSX domain		DNA probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_14_1750_s_155	10898790	( E,right gel) Major groove base modifications do not perturb binding of DSX domain to 15 base-pair DNA probe (5''-CACTACAATGTTGCA-3'' and complement): (lanes  e- g) single nebularine substitutions at positions 5, 7, and 8 of upper strand and (lanes  h- j) single 5-methylcytosine or uridine substituitions at positions 6, 9, and 11 of upper strand.	bind
3168	2	2109	6	10	NULL	0	NULL	major groove 		base modifications of	have no effect on					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_14_1750_s_155	10898790	( E,right gel) Major groove base modifications do not perturb binding of DSX domain to 15 base-pair DNA probe (5''-CACTACAATGTTGCA-3'' and complement): (lanes  e- g) single nebularine substitutions at positions 5, 7, and 8 of upper strand and (lanes  h- j) single 5-methylcytosine or uridine substituitions at positions 6, 9, and 11 of upper strand.	bind
4901	1	2109	7	10	NULL	0	NULL				binds			DSX domain 		DNA probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_14_1750_s_155	10898790	( E,right gel) Major groove base modifications do not perturb binding of DSX domain to 15 base-pair DNA probe (5''-CACTACAATGTTGCA-3'' and complement): (lanes  e- g) single nebularine substitutions at positions 5, 7, and 8 of upper strand and (lanes  h- j) single 5-methylcytosine or uridine substituitions at positions 6, 9, and 11 of upper strand.	bind
4903	2	2109	7	10	NULL	0	NULL	major groove		base modifications of	do not perturb					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_14_1750_s_155	10898790	( E,right gel) Major groove base modifications do not perturb binding of DSX domain to 15 base-pair DNA probe (5''-CACTACAATGTTGCA-3'' and complement): (lanes  e- g) single nebularine substitutions at positions 5, 7, and 8 of upper strand and (lanes  h- j) single 5-methylcytosine or uridine substituitions at positions 6, 9, and 11 of upper strand.	bind
3169	1	2110	6	10	NULL	0	NULL	GFP-alpha-CaMKII	GP		bind					calmodulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5411_162_s_107	10102820	( F) A GFP-alpha-CaMKII mutant deficient in calmodulin binding (A302R) fails to translocate to PSDs [same protocol as in (D)].	bind
3170	2	2110	6	10	NULL	0	NULL	GFP-alpha-CaMKII	GP		translocate to					PSDs	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5411_162_s_107	10102820	( F) A GFP-alpha-CaMKII mutant deficient in calmodulin binding (A302R) fails to translocate to PSDs [same protocol as in (D)].	bind
3171	3	2110	6	10	NULL	0	NULL	GFP-alpha-CaMKII	GP	mutant	does not bind			A302R		calmodulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5411_162_s_107	10102820	( F) A GFP-alpha-CaMKII mutant deficient in calmodulin binding (A302R) fails to translocate to PSDs [same protocol as in (D)].	bind
46297	4	2110	6	10	NULL	0	NULL	GFP-alpha-CaMKII	GP	mutant	inhibits			A302R		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5411_162_s_107	10102820	( F) A GFP-alpha-CaMKII mutant deficient in calmodulin binding (A302R) fails to translocate to PSDs [same protocol as in (D)].	bind
4910	1	2110	7	10	NULL	0	NULL	GFP-alpha-CaMKII	GP	mutant	does not bind			A302R		calmodulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5411_162_s_107	10102820	( F) A GFP-alpha-CaMKII mutant deficient in calmodulin binding (A302R) fails to translocate to PSDs [same protocol as in (D)].	bind
4912	2	2110	7	10	NULL	0	NULL	GFP-alpha-CaMKII	GP		translocate to					PSDs	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5411_162_s_107	10102820	( F) A GFP-alpha-CaMKII mutant deficient in calmodulin binding (A302R) fails to translocate to PSDs [same protocol as in (D)].	bind
46298	3	2110	7	10	NULL	0	NULL	GFP-alpha-CaMKII	GP	mutant	inhibit			A302R		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5411_162_s_107	10102820	( F) A GFP-alpha-CaMKII mutant deficient in calmodulin binding (A302R) fails to translocate to PSDs [same protocol as in (D)].	bind
3172	1	2111	6	10	NULL	0	NULL	EDA-A1	GP		bind					EDAR	GP				NULL	MCF7 cells	NULL	NULL	NULL	NULL	gw60_science_290_5491_523_s_98	11039935	( F) Binding of  EDA-A1 to EDAR results in activation of NF-kappaB in MCF7 cells.	bind
3173	2	2111	6	10	NULL	0	NULL	statement 1	Process		activates					NF-kappaB	GP				NULL	MCF7 cells	NULL	NULL	NULL	NULL	gw60_science_290_5491_523_s_98	11039935	( F) Binding of  EDA-A1 to EDAR results in activation of NF-kappaB in MCF7 cells.	bind
4916	1	2111	7	10	NULL	0	NULL	EDA-A1	GP		binds					EDAR	GP				NULL	in MCF7 cells	NULL	NULL	NULL	NULL	gw60_science_290_5491_523_s_98	11039935	( F) Binding of  EDA-A1 to EDAR results in activation of NF-kappaB in MCF7 cells.	bind
4917	2	2111	7	10	NULL	0	NULL	statement 1	Process		activates					NF-kappaB	GP				NULL	in MCF7 cells	NULL	NULL	NULL	NULL	gw60_science_290_5491_523_s_98	11039935	( F) Binding of  EDA-A1 to EDAR results in activation of NF-kappaB in MCF7 cells.	bind
3174	1	2112	6	10	NULL	0	NULL	ARF	GP		bind					Mix.2	GP	Xenopus		activin-response element of the promoter	NULL		NULL	NULL	NULL	NULL	gw60_science_298_5600_1996_s_100	12471260	( F) Binding of a FoxH1-Smad2-Smad4 transcription factor complex (ARF) to the activin-response element from the Xenopus  Mix.2 promoter ( 25) is inhibited by addition of DRAP1 in an electrophoretic mobility shift assay, whereas Dr1 has little or no effect; addition of antibodies to Smad2 (fig. S3) or to Smad4 supershifts the FoxH1-Smad2-Smad4 complex.	bind
3175	2	2112	6	10	NULL	0	NULL	ARF	GP		is					FoxH1-Smad2-Smad4 transcription factor complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_298_5600_1996_s_100	12471260	( F) Binding of a FoxH1-Smad2-Smad4 transcription factor complex (ARF) to the activin-response element from the Xenopus  Mix.2 promoter ( 25) is inhibited by addition of DRAP1 in an electrophoretic mobility shift assay, whereas Dr1 has little or no effect; addition of antibodies to Smad2 (fig. S3) or to Smad4 supershifts the FoxH1-Smad2-Smad4 complex.	bind
3176	3	2112	6	10	NULL	0	NULL	DRAP1	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_298_5600_1996_s_100	12471260	( F) Binding of a FoxH1-Smad2-Smad4 transcription factor complex (ARF) to the activin-response element from the Xenopus  Mix.2 promoter ( 25) is inhibited by addition of DRAP1 in an electrophoretic mobility shift assay, whereas Dr1 has little or no effect; addition of antibodies to Smad2 (fig. S3) or to Smad4 supershifts the FoxH1-Smad2-Smad4 complex.	bind
3177	4	2112	6	10	NULL	0	NULL	Dr1	GP		effect		may			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_298_5600_1996_s_100	12471260	( F) Binding of a FoxH1-Smad2-Smad4 transcription factor complex (ARF) to the activin-response element from the Xenopus  Mix.2 promoter ( 25) is inhibited by addition of DRAP1 in an electrophoretic mobility shift assay, whereas Dr1 has little or no effect; addition of antibodies to Smad2 (fig. S3) or to Smad4 supershifts the FoxH1-Smad2-Smad4 complex.	bind
4918	1	2112	7	10	NULL	0	NULL	FoxH1-Smad2-Smad4 transcription factor complex 	GP		binds					Mix.2	GP	Xenopus		activin-response element promoter of	NULL		NULL	NULL	NULL	NULL	gw60_science_298_5600_1996_s_100	12471260	( F) Binding of a FoxH1-Smad2-Smad4 transcription factor complex (ARF) to the activin-response element from the Xenopus  Mix.2 promoter ( 25) is inhibited by addition of DRAP1 in an electrophoretic mobility shift assay, whereas Dr1 has little or no effect; addition of antibodies to Smad2 (fig. S3) or to Smad4 supershifts the FoxH1-Smad2-Smad4 complex.	bind
4919	2	2112	7	10	NULL	0	NULL	DRAP1	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_298_5600_1996_s_100	12471260	( F) Binding of a FoxH1-Smad2-Smad4 transcription factor complex (ARF) to the activin-response element from the Xenopus  Mix.2 promoter ( 25) is inhibited by addition of DRAP1 in an electrophoretic mobility shift assay, whereas Dr1 has little or no effect; addition of antibodies to Smad2 (fig. S3) or to Smad4 supershifts the FoxH1-Smad2-Smad4 complex.	bind
4920	3	2112	7	10	NULL	0	NULL	Dr1	GP		effect		may			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_298_5600_1996_s_100	12471260	( F) Binding of a FoxH1-Smad2-Smad4 transcription factor complex (ARF) to the activin-response element from the Xenopus  Mix.2 promoter ( 25) is inhibited by addition of DRAP1 in an electrophoretic mobility shift assay, whereas Dr1 has little or no effect; addition of antibodies to Smad2 (fig. S3) or to Smad4 supershifts the FoxH1-Smad2-Smad4 complex.	bind
4922	4	2112	7	10	NULL	0	NULL	FoxH1-Smad2-Smad4 transcription factor complex	GP		is					ARF	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_298_5600_1996_s_100	12471260	( F) Binding of a FoxH1-Smad2-Smad4 transcription factor complex (ARF) to the activin-response element from the Xenopus  Mix.2 promoter ( 25) is inhibited by addition of DRAP1 in an electrophoretic mobility shift assay, whereas Dr1 has little or no effect; addition of antibodies to Smad2 (fig. S3) or to Smad4 supershifts the FoxH1-Smad2-Smad4 complex.	bind
3178	1	2113	6	10	NULL	0	NULL	NFAT1	GP		bind					TRAP gene	GP			NFAT binding element in promoter	NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_4_475_s_154	15314684	( F) Binding of NFAT1 to NFAT-binding element present in TRAP gene promoter ( - 523 to   - 507).	bind
46272	2	2113	6	10	NULL	0	NULL				is present in				NFAT-binding element	TRAP gene	GP			- 523 to - 507 of promoter	NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_4_475_s_154	15314684	( F) Binding of NFAT1 to NFAT-binding element present in TRAP gene promoter ( - 523 to   - 507).	bind
4923	1	2113	7	10	NULL	0	NULL	NFAT1	GP		binds					TRAP gene	GP			 NFAT-binding element in promoter	NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_4_475_s_154	15314684	( F) Binding of NFAT1 to NFAT-binding element present in TRAP gene promoter ( - 523 to   - 507).	bind
4924	2	2113	7	10	NULL	0	NULL				is present in				 NFAT-binding element 	TRAP gene	GP			 - 523 to - 507 promoter	NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_114_4_475_s_154	15314684	( F) Binding of NFAT1 to NFAT-binding element present in TRAP gene promoter ( - 523 to   - 507).	bind
3199	1	2114	6	10	NULL	0	NULL	menin	GP	wild type	bind									p27Kip1 locus	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_3_749_s_142	15640349	( F) Binding of the menin mutants L22R (gray) and A242V (red) are reduced at the  p27Kip1 and  p18Ink4c loci compared with wild-type menin ( Men1-/- with reexpressed menin, green).	bind
3212	2	2114	6	10	NULL	0	NULL	menin	GP	mutant	bind			L22R						p27Kip1 locus	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_3_749_s_142	15640349	( F) Binding of the menin mutants L22R (gray) and A242V (red) are reduced at the  p27Kip1 and  p18Ink4c loci compared with wild-type menin ( Men1-/- with reexpressed menin, green).	bind
3213	3	2114	6	10	NULL	0	NULL	statement 2	Process		is reduced than					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_3_749_s_142	15640349	( F) Binding of the menin mutants L22R (gray) and A242V (red) are reduced at the  p27Kip1 and  p18Ink4c loci compared with wild-type menin ( Men1-/- with reexpressed menin, green).	bind
3214	5	2114	6	10	NULL	0	NULL	menin	GP	wild type	bind									p18Ink4c loci	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_3_749_s_142	15640349	( F) Binding of the menin mutants L22R (gray) and A242V (red) are reduced at the  p27Kip1 and  p18Ink4c loci compared with wild-type menin ( Men1-/- with reexpressed menin, green).	bind
3645	4	2114	6	10	NULL	0	NULL	menin	GP	mutant	bind			A242V						p27Kip1 locus	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_3_749_s_142	15640349	( F) Binding of the menin mutants L22R (gray) and A242V (red) are reduced at the  p27Kip1 and  p18Ink4c loci compared with wild-type menin ( Men1-/- with reexpressed menin, green).	bind
3646	6	2114	6	10	NULL	0	NULL	statement 4	Process		is reduced than					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_3_749_s_142	15640349	( F) Binding of the menin mutants L22R (gray) and A242V (red) are reduced at the  p27Kip1 and  p18Ink4c loci compared with wild-type menin ( Men1-/- with reexpressed menin, green).	bind
3647	7	2114	6	10	NULL	0	NULL	menin	GP	mutant	bind			A242V						p18Ink4c loci	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_3_749_s_142	15640349	( F) Binding of the menin mutants L22R (gray) and A242V (red) are reduced at the  p27Kip1 and  p18Ink4c loci compared with wild-type menin ( Men1-/- with reexpressed menin, green).	bind
3648	8	2114	6	10	NULL	0	NULL	statement 7	Process		is reduced than					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_3_749_s_142	15640349	( F) Binding of the menin mutants L22R (gray) and A242V (red) are reduced at the  p27Kip1 and  p18Ink4c loci compared with wild-type menin ( Men1-/- with reexpressed menin, green).	bind
3649	9	2114	6	10	NULL	0	NULL	menin	GP	mutant	bind			L22R						p18Ink4c loci	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_3_749_s_142	15640349	( F) Binding of the menin mutants L22R (gray) and A242V (red) are reduced at the  p27Kip1 and  p18Ink4c loci compared with wild-type menin ( Men1-/- with reexpressed menin, green).	bind
3650	10	2114	6	10	NULL	0	NULL	statement 9	Process		is reduced than					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_3_749_s_142	15640349	( F) Binding of the menin mutants L22R (gray) and A242V (red) are reduced at the  p27Kip1 and  p18Ink4c loci compared with wild-type menin ( Men1-/- with reexpressed menin, green).	bind
4935	1	2114	7	10	NULL	0	NULL	menin	GP	Wild-type	binds									p27Kip1 locus	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_3_749_s_142	15640349	( F) Binding of the menin mutants L22R (gray) and A242V (red) are reduced at the  p27Kip1 and  p18Ink4c loci compared with wild-type menin ( Men1-/- with reexpressed menin, green).	bind
4936	2	2114	7	10	NULL	0	NULL	menin	GP	Wild-type	binds									p18Ink4c locus	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_3_749_s_142	15640349	( F) Binding of the menin mutants L22R (gray) and A242V (red) are reduced at the  p27Kip1 and  p18Ink4c loci compared with wild-type menin ( Men1-/- with reexpressed menin, green).	bind
4937	3	2114	7	10	NULL	0	NULL	menin	GP	mutant	binds			L22R						p27Kip1 locus	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_3_749_s_142	15640349	( F) Binding of the menin mutants L22R (gray) and A242V (red) are reduced at the  p27Kip1 and  p18Ink4c loci compared with wild-type menin ( Men1-/- with reexpressed menin, green).	bind
4942	4	2114	7	10	NULL	0	NULL	menin	GP	mutant	binds			L22R						p18Ink4c locus	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_3_749_s_142	15640349	( F) Binding of the menin mutants L22R (gray) and A242V (red) are reduced at the  p27Kip1 and  p18Ink4c loci compared with wild-type menin ( Men1-/- with reexpressed menin, green).	bind
4946	5	2114	7	10	NULL	0	NULL	menin	GP	mutant	binds			A242V						p27Kip1 locus	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_3_749_s_142	15640349	( F) Binding of the menin mutants L22R (gray) and A242V (red) are reduced at the  p27Kip1 and  p18Ink4c loci compared with wild-type menin ( Men1-/- with reexpressed menin, green).	bind
4947	6	2114	7	10	NULL	0	NULL	menin	GP	mutant	binds			A242V						p18Ink4c locus	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_3_749_s_142	15640349	( F) Binding of the menin mutants L22R (gray) and A242V (red) are reduced at the  p27Kip1 and  p18Ink4c loci compared with wild-type menin ( Men1-/- with reexpressed menin, green).	bind
4957	7	2114	7	10	NULL	0	NULL	statement 3	Process		is reduced than					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_3_749_s_142	15640349	( F) Binding of the menin mutants L22R (gray) and A242V (red) are reduced at the  p27Kip1 and  p18Ink4c loci compared with wild-type menin ( Men1-/- with reexpressed menin, green).	bind
6239	8	2114	7	10	NULL	0	NULL	statement 4	Process		is reduced than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_3_749_s_142	15640349	( F) Binding of the menin mutants L22R (gray) and A242V (red) are reduced at the  p27Kip1 and  p18Ink4c loci compared with wild-type menin ( Men1-/- with reexpressed menin, green).	bind
6241	9	2114	7	10	NULL	0	NULL	statement 5	Process		is reduced than					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_3_749_s_142	15640349	( F) Binding of the menin mutants L22R (gray) and A242V (red) are reduced at the  p27Kip1 and  p18Ink4c loci compared with wild-type menin ( Men1-/- with reexpressed menin, green).	bind
6243	10	2114	7	10	NULL	0	NULL	statement 6	Process		is reduced than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_3_749_s_142	15640349	( F) Binding of the menin mutants L22R (gray) and A242V (red) are reduced at the  p27Kip1 and  p18Ink4c loci compared with wild-type menin ( Men1-/- with reexpressed menin, green).	bind
3179	1	2116	6	10	NULL	0	NULL	Ebp1	GP		bind			N-terminus		Akt	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_10_2083_s_153	16642037	( F) Both N- and C-termini of Ebp1 bind to Akt.	bind
3180	2	2116	6	10	NULL	0	NULL	Ebp1	GP		bind			C-terminus		Akt	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_10_2083_s_153	16642037	( F) Both N- and C-termini of Ebp1 bind to Akt.	bind
4958	1	2116	7	10	NULL	0	NULL	Ebp1 	GP		binds			N terminus		Akt	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_10_2083_s_153	16642037	( F) Both N- and C-termini of Ebp1 bind to Akt.	bind
4959	2	2116	7	10	NULL	0	NULL	Ebp1 	GP		binds			C terminus		Akt	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_10_2083_s_153	16642037	( F) Both N- and C-termini of Ebp1 bind to Akt.	bind
3181	1	2117	6	10	NULL	0	NULL	p27	GP		bind					Cdk2	GP				NULL	Bosc23 cells	NULL	NULL	NULL	NULL	gw60_jclininvest_104_7_865_s_195	10510327	( f) Cdk2 immunoprecipitates in Bosc23 cells: p27 bound to Cdk2, Cdk2 level, and Cdk2 activity in total or fractionated extracts.	bind
4960	1	2117	7	10	NULL	0	NULL	p27	GP		binds					Cdk2	GP				NULL	Bosc23 cells	NULL	NULL	NULL	NULL	gw60_jclininvest_104_7_865_s_195	10510327	( f) Cdk2 immunoprecipitates in Bosc23 cells: p27 bound to Cdk2, Cdk2 level, and Cdk2 activity in total or fractionated extracts.	bind
3209	1	2119	6	10	NULL	0	NULL	Srb4-Myc	GP		bind					GAL1	GP			UASG	NULL	yeast cells	NULL	NULL	NULL	NULL	gw70_embo_23_20_4040_s_153	15385957	( F) ChIP analysis of the binding of Srb4-Myc and Rpb1 to the  GAL1 UASG in yeast cells expressing a Gal4-Gal11 fusion (KLY091 and KLY092).	bind
3210	2	2119	6	10	NULL	0	NULL	Rbp1	GP		bind					GAL1	GP			UASG	NULL	yeast cells	NULL	NULL	NULL	NULL	gw70_embo_23_20_4040_s_153	15385957	( F) ChIP analysis of the binding of Srb4-Myc and Rpb1 to the  GAL1 UASG in yeast cells expressing a Gal4-Gal11 fusion (KLY091 and KLY092).	bind
3211	3	2119	6	10	NULL	0	NULL	yeast cells 	Cell		express					Gal4-Gal11	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_20_4040_s_153	15385957	( F) ChIP analysis of the binding of Srb4-Myc and Rpb1 to the  GAL1 UASG in yeast cells expressing a Gal4-Gal11 fusion (KLY091 and KLY092).	bind
46138	4	2119	6	10	NULL	0	NULL	Gal4-Gal11	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_20_4040_s_153	15385957	( F) ChIP analysis of the binding of Srb4-Myc and Rpb1 to the  GAL1 UASG in yeast cells expressing a Gal4-Gal11 fusion (KLY091 and KLY092).	bind
4961	1	2119	7	10	NULL	0	NULL	Srb4-Myc	GP		bind					GAL1	GP			UASG	NULL	yeast cells	NULL	NULL	NULL	NULL	gw70_embo_23_20_4040_s_153	15385957	( F) ChIP analysis of the binding of Srb4-Myc and Rpb1 to the  GAL1 UASG in yeast cells expressing a Gal4-Gal11 fusion (KLY091 and KLY092).	bind
4962	2	2119	7	10	NULL	0	NULL	Rpb1	GP		bind					GAL1 	GP			UASG	NULL	yeast cells	NULL	NULL	NULL	NULL	gw70_embo_23_20_4040_s_153	15385957	( F) ChIP analysis of the binding of Srb4-Myc and Rpb1 to the  GAL1 UASG in yeast cells expressing a Gal4-Gal11 fusion (KLY091 and KLY092).	bind
46139	4	2119	7	10	NULL	0	NULL	Gal4-Gal11	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_20_4040_s_153	15385957	( F) ChIP analysis of the binding of Srb4-Myc and Rpb1 to the  GAL1 UASG in yeast cells expressing a Gal4-Gal11 fusion (KLY091 and KLY092).	bind
46283	3	2119	7	10	NULL	0	NULL	yeast cells	Cell		express					Gal4-Gal11	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_20_4040_s_153	15385957	( F) ChIP analysis of the binding of Srb4-Myc and Rpb1 to the  GAL1 UASG in yeast cells expressing a Gal4-Gal11 fusion (KLY091 and KLY092).	bind
3182	1	2121	6	10	NULL	0	NULL	NFAT	GP		bind					ARRE2	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_5_1081_s_108	16498406	( F) CpG site 1 methylation inhibits NFAT and Oct-1 binding to ARRE2.	bind
3183	2	2121	6	10	NULL	0	NULL	Oct-1	GP		bind					ARRE2	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_5_1081_s_108	16498406	( F) CpG site 1 methylation inhibits NFAT and Oct-1 binding to ARRE2.	bind
3184	3	2121	6	10	NULL	0	NULL	CpG	GP	methylation	inhibits				site 1	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_5_1081_s_108	16498406	( F) CpG site 1 methylation inhibits NFAT and Oct-1 binding to ARRE2.	bind
3185	4	2121	6	10	NULL	0	NULL	CpG	GP	methylation	inhibits				site 1	statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_5_1081_s_108	16498406	( F) CpG site 1 methylation inhibits NFAT and Oct-1 binding to ARRE2.	bind
4965	1	2121	7	10	NULL	0	NULL	NFAT	GP		binds					ARRE2	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_5_1081_s_108	16498406	( F) CpG site 1 methylation inhibits NFAT and Oct-1 binding to ARRE2.	bind
4966	2	2121	7	10	NULL	0	NULL	Oct-1	GP		binds					ARRE2	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_5_1081_s_108	16498406	( F) CpG site 1 methylation inhibits NFAT and Oct-1 binding to ARRE2.	bind
4967	3	2121	7	10	NULL	0	NULL	CpG 	GP	methylation 	inhibits				site 1	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_5_1081_s_108	16498406	( F) CpG site 1 methylation inhibits NFAT and Oct-1 binding to ARRE2.	bind
4968	4	2121	7	10	NULL	0	NULL	CpG 	GP	methylation	inhibits				site 1	statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_5_1081_s_108	16498406	( F) CpG site 1 methylation inhibits NFAT and Oct-1 binding to ARRE2.	bind
3251	1	2122	6	10	NULL	0	NULL	Myc	GP	endogenous	bind		directly							hGCN5 locus	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_embo_25_12_2723_s_98	16724113	( F) Direct binding of endogenous Myc to the hGCN5 locus  in vivo.	bind
4969	1	2122	7	10	NULL	0	NULL	Myc	GP	endogenous	binds to		directly							hGCN5 locus	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_embo_25_12_2723_s_98	16724113	( F) Direct binding of endogenous Myc to the hGCN5 locus  in vivo.	bind
3252	1	2123	6	10	NULL	0	NULL	TLX	GP		bind		directly			Pten	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_20_10_1308_s_161	16702404	( F) Direct binding of TLX to the  Pten promoter region in gel shift assays.	bind
4970	1	2123	7	10	NULL	0	NULL	TLX 	GP		binds to		directly			Pten	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_20_10_1308_s_161	16702404	( F) Direct binding of TLX to the  Pten promoter region in gel shift assays.	bind
3253	1	2125	6	10	NULL	0	NULL	Spn-F	GP		bind					GST-Ddlc	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_development_133_8_1477_s_222	16540510	( F) In vitro binding of Spn-F to GST-Ddlc.	bind
4972	1	2125	7	10	NULL	0	NULL	Spn-F	GP		binds					GST-Ddlc	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_development_133_8_1477_s_222	16540510	( F) In vitro binding of Spn-F to GST-Ddlc.	bind
3254	1	2126	6	10	NULL	0	NULL	Prp 	GP		does not bind			27-30		HDL particles	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_30_11312_s_67	16849426	( F) Incubation of PrP 27 - 30 with HDL shows that virtually no HDL particles bind to  the prion rods.	bind
4973	1	2126	7	10	NULL	0	NULL	HDL	Chemical		does not bind					PrP	GP		27 - 30		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_30_11312_s_67	16849426	( F) Incubation of PrP 27 - 30 with HDL shows that virtually no HDL particles bind to  the prion rods.	bind
3255	1	2128	6	10	NULL	0	NULL	Imp4 	GP		bind		weakly			U3 MINI	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_43_15301_s_127	15489263	( F) Nondenaturing PAGE shows that the Imp4 core protein binds weakly to U3 MINI but  does not promote formation of the U3 - ETS duplex.	bind
3256	2	2128	6	10	NULL	0	NULL	Imp4	GP		does not promote 					U3 - ETS duplex	NucleicAcid	formation of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_43_15301_s_127	15489263	( F) Nondenaturing PAGE shows that the Imp4 core protein binds weakly to U3 MINI but  does not promote formation of the U3 - ETS duplex.	bind
46300	3	2128	6	10	NULL	0	NULL	Imp4	GP		is a type of					core protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_43_15301_s_127	15489263	( F) Nondenaturing PAGE shows that the Imp4 core protein binds weakly to U3 MINI but  does not promote formation of the U3 - ETS duplex.	bind
4974	1	2128	7	10	NULL	0	NULL	Imp4	GP		binds		weakly			U3 MINI	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_43_15301_s_127	15489263	( F) Nondenaturing PAGE shows that the Imp4 core protein binds weakly to U3 MINI but  does not promote formation of the U3 - ETS duplex.	bind
4975	2	2128	7	10	NULL	0	NULL	Imp4	GP		does not promote					U3 - ETS duplex	NucleicAcid	formation of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_43_15301_s_127	15489263	( F) Nondenaturing PAGE shows that the Imp4 core protein binds weakly to U3 MINI but  does not promote formation of the U3 - ETS duplex.	bind
46299	3	2128	7	10	NULL	0	NULL	Imp4	GP		is a type of					core protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_43_15301_s_127	15489263	( F) Nondenaturing PAGE shows that the Imp4 core protein binds weakly to U3 MINI but  does not promote formation of the U3 - ETS duplex.	bind
3257	1	2129	6	10	NULL	0	NULL	p97	GP		bind					eIF2beta	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_embo_25_17_4008_s_72	16932749	( F) p97 binds eIF2beta in vivo.	bind
4976	1	2129	7	10	NULL	0	NULL	 p97	GP		binds					eIF2beta	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_embo_25_17_4008_s_72	16932749	( F) p97 binds eIF2beta in vivo.	bind
3258	1	2130	6	10	NULL	0	NULL	PTG	GP		bind					phosphorylase kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_275_5305_1475_s_62	9045612	( F) PTG binds phosphorylase kinase.	bind
4977	1	2130	7	10	NULL	0	NULL	PTG	GP		binds					phosphorylase kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_275_5305_1475_s_62	9045612	( F) PTG binds phosphorylase kinase.	bind
3259	1	2131	6	10	NULL	0	NULL	AQP1-specific antibody	GP		bind					AQP1	GP		carboxyl domain 		NULL	ZG membrane intragranular side	NULL	NULL	NULL	NULL	gw60_pnas_99_7_4720_s_161	11917120	( F) Schematic diagram of ZG membrane depicting AQP1-specific antibody binding to the carboxyl domain of AQP1 at the intragranular side to block water gating.	bind
46192	2	2131	6	10	NULL	0	NULL	statement 1	Process		blocks					water gating	Process				NULL	ZG membrane intragranular side	NULL	NULL	NULL	NULL	gw60_pnas_99_7_4720_s_161	11917120	( F) Schematic diagram of ZG membrane depicting AQP1-specific antibody binding to the carboxyl domain of AQP1 at the intragranular side to block water gating.	bind
4978	1	2131	7	10	NULL	0	NULL	AQP1-specific antibody	GP		binds to 					AQP1	GP		 carboxyl domain		NULL	ZG membrane intragranular side	NULL	NULL	NULL	NULL	gw60_pnas_99_7_4720_s_161	11917120	( F) Schematic diagram of ZG membrane depicting AQP1-specific antibody binding to the carboxyl domain of AQP1 at the intragranular side to block water gating.	bind
4980	3	2131	7	10	NULL	0	NULL	statement 1	Process		blocks					water gating	Process				NULL	ZG membrane intragranular side	NULL	NULL	NULL	NULL	gw60_pnas_99_7_4720_s_161	11917120	( F) Schematic diagram of ZG membrane depicting AQP1-specific antibody binding to the carboxyl domain of AQP1 at the intragranular side to block water gating.	bind
3260	1	2133	6	10	NULL	0	NULL	HVEM-Fc	GP		bind					BTLA-Fc	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_4_1116_s_135	15647361	( F) Sensorgrams of HVEM-Fc (10 nM) binding to immobilized BTLA-Fc in the presence of  increasing amounts of gD (delta290 - 299).	bind
3261	2	2133	6	10	NULL	0	NULL	statement 1	Process		in presence of 					gD	GP	increasing amounts of	delta290 - 299		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_4_1116_s_135	15647361	( F) Sensorgrams of HVEM-Fc (10 nM) binding to immobilized BTLA-Fc in the presence of  increasing amounts of gD (delta290 - 299).	bind
4981	1	2133	7	10	NULL	0	NULL	HVEM-Fc	GP		binds to					BTLA-Fc 	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_4_1116_s_135	15647361	( F) Sensorgrams of HVEM-Fc (10 nM) binding to immobilized BTLA-Fc in the presence of  increasing amounts of gD (delta290 - 299).	bind
4982	2	2133	7	10	NULL	0	NULL	statement 1	Process		occurs in the presence					 gD	GP	increasing amounts of	delta290 - 299		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_4_1116_s_135	15647361	( F) Sensorgrams of HVEM-Fc (10 nM) binding to immobilized BTLA-Fc in the presence of  increasing amounts of gD (delta290 - 299).	bind
3262	1	2134	6	10	NULL	0	NULL	MukF	GP	tagged	bind			331-440		MukB	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_11_1921_s_142	15902272	( F) Tagged MukF(331 440) binds MukB.	bind
4984	1	2134	7	10	NULL	0	NULL	MukF	GP	Tagged	binds			331-440		MukB	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_11_1921_s_142	15902272	( F) Tagged MukF(331 440) binds MukB.	bind
3263	1	2135	6	10	NULL	0	NULL	c-Src	GP		bind					nAchRs	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_8_2208_s_129	16862215	( F) The binding between c-Src and nAChRs was inhibited by the Src inhibitor PP2.	bind
3264	2	2135	6	10	NULL	0	NULL	PP2	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_8_2208_s_129	16862215	( F) The binding between c-Src and nAChRs was inhibited by the Src inhibitor PP2.	bind
45892	3	2135	6	10	NULL	0	NULL	PP2	GP		is a type of					Src inhibitor	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_8_2208_s_129	16862215	( F) The binding between c-Src and nAChRs was inhibited by the Src inhibitor PP2.	bind
4985	1	2135	7	10	NULL	0	NULL	c-Src	GP		binds					nAChRs	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_8_2208_s_129	16862215	( F) The binding between c-Src and nAChRs was inhibited by the Src inhibitor PP2.	bind
4986	2	2135	7	10	NULL	0	NULL	statement 1	Process		is inhibited by					PP2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_8_2208_s_129	16862215	( F) The binding between c-Src and nAChRs was inhibited by the Src inhibitor PP2.	bind
45893	3	2135	7	10	NULL	0	NULL	PP2	GP		is a type of					Src inhibitor	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_8_2208_s_129	16862215	( F) The binding between c-Src and nAChRs was inhibited by the Src inhibitor PP2.	bind
3265	1	2136	6	10	NULL	0	NULL	IE2	GP	mutant	bind					p53/p300 complex	GP	endogenous			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_11_2269_s_192	15141169	( F) The HAT inhibition mutant of IE2 binds to the endogenous p53/p300 complex on the   p21 promoter.	bind
3266	2	2136	6	10	NULL	0	NULL	IE2	GP	mutant	inhibits					HAT	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_11_2269_s_192	15141169	( F) The HAT inhibition mutant of IE2 binds to the endogenous p53/p300 complex on the   p21 promoter.	bind
45897	3	2136	6	10	NULL	0	NULL	statement 1	Process		occurs in					p21	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_embo_23_11_2269_s_192	15141169	( F) The HAT inhibition mutant of IE2 binds to the endogenous p53/p300 complex on the   p21 promoter.	bind
5104	1	2136	7	10	NULL	0	NULL	IE2	GP	mutant	binds to					 p53/p300 complex	GP	endogenous			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_11_2269_s_192	15141169	( F) The HAT inhibition mutant of IE2 binds to the endogenous p53/p300 complex on the   p21 promoter.	bind
5106	2	2136	7	10	NULL	0	NULL	statement 1	Process		occurs in 					p21	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_embo_23_11_2269_s_192	15141169	( F) The HAT inhibition mutant of IE2 binds to the endogenous p53/p300 complex on the   p21 promoter.	bind
45896	3	2136	7	10	NULL	0	NULL	IE2	GP	mutant	inhibit					HAT	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_11_2269_s_192	15141169	( F) The HAT inhibition mutant of IE2 binds to the endogenous p53/p300 complex on the   p21 promoter.	bind
3291	1	2137	6	10	NULL	0	NULL	TMEFF1	GP	mutant	bind			follistatin modules		Cripto	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_21_2624_s_134	14563676	( F) The TMEFF1 deletion mutants that lack either the follistatin modules or the EGF  motif still bind to Cripto.	bind
3292	2	2137	6	10	NULL	0	NULL	TMEFF1	GP	mutant	bind			EGF motif		Cripto	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_21_2624_s_134	14563676	( F) The TMEFF1 deletion mutants that lack either the follistatin modules or the EGF  motif still bind to Cripto.	bind
5107	1	2137	7	10	NULL	0	NULL	 TMEFF1 	GP	mutant	binds			follistatin modules		Cripto	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_21_2624_s_134	14563676	( F) The TMEFF1 deletion mutants that lack either the follistatin modules or the EGF  motif still bind to Cripto.	bind
5108	2	2137	7	10	NULL	0	NULL	TMEFF1	GP	mutant	binds			EGF motif		Cripto	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_21_2624_s_134	14563676	( F) The TMEFF1 deletion mutants that lack either the follistatin modules or the EGF  motif still bind to Cripto.	bind
3293	1	2138	6	10	NULL	0	NULL	progesterone	GP		bind		specifically			mPRgamma	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_5_2237_s_156	12601167	( f) Time course of association and dissociation of specific progesterone binding to  human mPRgamma.	bind
5109	1	2138	7	10	NULL	0	NULL	progesterone	GP		binds to		specifically			mPRgamma	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_5_2237_s_156	12601167	( f) Time course of association and dissociation of specific progesterone binding to  human mPRgamma.	bind
3294	1	2140	6	10	NULL	0	NULL				bind			V3IIIB		Fv	GP		residues T303		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_38_13950_s_92	16966601	( F) V3IIIB bound to 0.5beta Fv; residues T303 and K322, not included in the NMR structure, were modeled.	bind
3295	2	2140	6	10	NULL	0	NULL				bind			V3IIIB		Fv	GP		residues K322		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_38_13950_s_92	16966601	( F) V3IIIB bound to 0.5beta Fv; residues T303 and K322, not included in the NMR structure, were modeled.	bind
5110	1	2140	7	10	NULL	0	NULL				bind			V3IIIB		 Fv	GP		residues T303		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_38_13950_s_92	16966601	( F) V3IIIB bound to 0.5beta Fv; residues T303 and K322, not included in the NMR structure, were modeled.	bind
46293	2	2140	7	10	NULL	0	NULL				bind			V3IIIB 		Fv	GP		residues K322		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_38_13950_s_92	16966601	( F) V3IIIB bound to 0.5beta Fv; residues T303 and K322, not included in the NMR structure, were modeled.	bind
3296	1	2141	6	10	NULL	0	NULL	Oct-1	GP		bind					SV40	GP			octamer element of enhancer	NULL	HeLa nuclear extracts	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_9_4575_s_239	7876228	( Fig. 6  B) Thus the predominant  complexes formed in HeLa nuclear extracts with this region of the SV40  enhancer contain Oct-1 bound to the octamer element and HIP116 bound  specifically to the SPH repeats.	bind
3297	2	2141	6	10	NULL	0	NULL	HIP116	GP		bind		specifically			SV40	GP			SPH repeats of enhancer	NULL	HeLa nuclear extracts	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_9_4575_s_239	7876228	( Fig. 6  B) Thus the predominant  complexes formed in HeLa nuclear extracts with this region of the SV40  enhancer contain Oct-1 bound to the octamer element and HIP116 bound  specifically to the SPH repeats.	bind
5111	1	2141	7	10	NULL	0	NULL	Oct-1	GP		binds					SV40	GP			octamer element of enhancer	NULL	HeLa nuclear extracts	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_9_4575_s_239	7876228	( Fig. 6  B) Thus the predominant  complexes formed in HeLa nuclear extracts with this region of the SV40  enhancer contain Oct-1 bound to the octamer element and HIP116 bound  specifically to the SPH repeats.	bind
5112	2	2141	7	10	NULL	0	NULL	HIP116	GP		binds		specifically			SV40	GP			SPH repeats of enhancer	NULL	HeLa nuclear extracts	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_9_4575_s_239	7876228	( Fig. 6  B) Thus the predominant  complexes formed in HeLa nuclear extracts with this region of the SV40  enhancer contain Oct-1 bound to the octamer element and HIP116 bound  specifically to the SPH repeats.	bind
3298	1	2142	6	10	NULL	0	NULL	TBL1	GP		bind					H2B	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_66_0_315_s_230	14977406	( Figures 3 and 5) ( 177, 180, 184, 189); TBL1 and TBLR1 also bind to histones H2B and H4 ( 189) and may help in chromatin substrate recognition.	bind
3299	2	2142	6	10	NULL	0	NULL	TBL1	GP		bind					H4	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_66_0_315_s_230	14977406	( Figures 3 and 5) ( 177, 180, 184, 189); TBL1 and TBLR1 also bind to histones H2B and H4 ( 189) and may help in chromatin substrate recognition.	bind
3300	3	2142	6	10	NULL	0	NULL	TBLR1	GP		bind					H2B	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_66_0_315_s_230	14977406	( Figures 3 and 5) ( 177, 180, 184, 189); TBL1 and TBLR1 also bind to histones H2B and H4 ( 189) and may help in chromatin substrate recognition.	bind
3301	4	2142	6	10	NULL	0	NULL	TBLR1	GP		bind					H4	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_66_0_315_s_230	14977406	( Figures 3 and 5) ( 177, 180, 184, 189); TBL1 and TBLR1 also bind to histones H2B and H4 ( 189) and may help in chromatin substrate recognition.	bind
3302	5	2142	6	10	NULL	0	NULL	TBL1	GP		help in		may			chromatin substrate	GP	recognition of			NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_66_0_315_s_230	14977406	( Figures 3 and 5) ( 177, 180, 184, 189); TBL1 and TBLR1 also bind to histones H2B and H4 ( 189) and may help in chromatin substrate recognition.	bind
3303	6	2142	6	10	NULL	0	NULL	TBLR1	GP		help in		may			chromatin substrate	GP	recognition of			NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_66_0_315_s_230	14977406	( Figures 3 and 5) ( 177, 180, 184, 189); TBL1 and TBLR1 also bind to histones H2B and H4 ( 189) and may help in chromatin substrate recognition.	bind
45902	7	2142	6	10	NULL	0	NULL	H2B	GP		is a type of					histone	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_66_0_315_s_230	14977406	( Figures 3 and 5) ( 177, 180, 184, 189); TBL1 and TBLR1 also bind to histones H2B and H4 ( 189) and may help in chromatin substrate recognition.	bind
45903	8	2142	6	10	NULL	0	NULL	H4	GP		is a type of					histone	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_66_0_315_s_230	14977406	( Figures 3 and 5) ( 177, 180, 184, 189); TBL1 and TBLR1 also bind to histones H2B and H4 ( 189) and may help in chromatin substrate recognition.	bind
5116	1	2142	7	10	NULL	0	NULL	TBL1	GP		binds					H2B	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_66_0_315_s_230	14977406	( Figures 3 and 5) ( 177, 180, 184, 189); TBL1 and TBLR1 also bind to histones H2B and H4 ( 189) and may help in chromatin substrate recognition.	bind
5117	2	2142	7	10	NULL	0	NULL	TBL1	GP		binds					H4	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_66_0_315_s_230	14977406	( Figures 3 and 5) ( 177, 180, 184, 189); TBL1 and TBLR1 also bind to histones H2B and H4 ( 189) and may help in chromatin substrate recognition.	bind
5118	3	2142	7	10	NULL	0	NULL	TBLR1	GP		binds					H2B	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_66_0_315_s_230	14977406	( Figures 3 and 5) ( 177, 180, 184, 189); TBL1 and TBLR1 also bind to histones H2B and H4 ( 189) and may help in chromatin substrate recognition.	bind
5119	4	2142	7	10	NULL	0	NULL	TBLR1	GP		binds					H4	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_66_0_315_s_230	14977406	( Figures 3 and 5) ( 177, 180, 184, 189); TBL1 and TBLR1 also bind to histones H2B and H4 ( 189) and may help in chromatin substrate recognition.	bind
5120	5	2142	7	10	NULL	0	NULL	statement 1	Process		helps in					chromatin substrate	GP	recognizing			NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_66_0_315_s_230	14977406	( Figures 3 and 5) ( 177, 180, 184, 189); TBL1 and TBLR1 also bind to histones H2B and H4 ( 189) and may help in chromatin substrate recognition.	bind
5121	6	2142	7	10	NULL	0	NULL	statement 2	Process		helps in					chromatin substrate	GP	recognizing			NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_66_0_315_s_230	14977406	( Figures 3 and 5) ( 177, 180, 184, 189); TBL1 and TBLR1 also bind to histones H2B and H4 ( 189) and may help in chromatin substrate recognition.	bind
5122	7	2142	7	10	NULL	0	NULL	statement 3	Process		helps in					chromatin substrate	GP	recognizing			NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_66_0_315_s_230	14977406	( Figures 3 and 5) ( 177, 180, 184, 189); TBL1 and TBLR1 also bind to histones H2B and H4 ( 189) and may help in chromatin substrate recognition.	bind
5123	8	2142	7	10	NULL	0	NULL	statement 4	Process		helps in					chromatin substrate	GP	recognizing			NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_66_0_315_s_230	14977406	( Figures 3 and 5) ( 177, 180, 184, 189); TBL1 and TBLR1 also bind to histones H2B and H4 ( 189) and may help in chromatin substrate recognition.	bind
45904	9	2142	7	10	NULL	0	NULL	H2B	GP		is a type of					histone	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_66_0_315_s_230	14977406	( Figures 3 and 5) ( 177, 180, 184, 189); TBL1 and TBLR1 also bind to histones H2B and H4 ( 189) and may help in chromatin substrate recognition.	bind
45905	10	2142	7	10	NULL	0	NULL	H4 \t	GP		is a type of					histone	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_66_0_315_s_230	14977406	( Figures 3 and 5) ( 177, 180, 184, 189); TBL1 and TBLR1 also bind to histones H2B and H4 ( 189) and may help in chromatin substrate recognition.	bind
3395	1	2143	6	10	NULL	0	NULL	p53	GP		bind					DNA	NucleicAcid				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_embo_23_11_2269_s_240	15141169	( Figures 3,  5, and  7), and that IE2 deletion mutants (aa 136 579 and 169 579) lacking the minimal N-terminal  HAT inhibitory domain failed to repress the  in vivo DNA binding of p53 and local histone acetylation ( Figures 1C,  5,  7E, F,  8, and  9).	bind
3396	2	2143	6	10	NULL	0	NULL	IE2	GP	deletion mutant	fail to repress			aa 136 579;;169 579		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_11_2269_s_240	15141169	( Figures 3,  5, and  7), and that IE2 deletion mutants (aa 136 579 and 169 579) lacking the minimal N-terminal  HAT inhibitory domain failed to repress the  in vivo DNA binding of p53 and local histone acetylation ( Figures 1C,  5,  7E, F,  8, and  9).	bind
3798	3	2143	6	10	NULL	0	NULL	IE2	GP	deletion mutant	lacks			aa 136 579;;169 579					minimal N-terminal HAT inhibitory domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_11_2269_s_240	15141169	( Figures 3,  5, and  7), and that IE2 deletion mutants (aa 136 579 and 169 579) lacking the minimal N-terminal  HAT inhibitory domain failed to repress the  in vivo DNA binding of p53 and local histone acetylation ( Figures 1C,  5,  7E, F,  8, and  9).	bind
3799	4	2143	6	10	NULL	0	NULL	IE2	GP	deletion mutant	fail to repress			aa 136 579;;169 579		histone	GP	acetylation of			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_11_2269_s_240	15141169	( Figures 3,  5, and  7), and that IE2 deletion mutants (aa 136 579 and 169 579) lacking the minimal N-terminal  HAT inhibitory domain failed to repress the  in vivo DNA binding of p53 and local histone acetylation ( Figures 1C,  5,  7E, F,  8, and  9).	bind
5124	1	2143	7	10	NULL	0	NULL	p53	GP		binds					DNA	NucleicAcid				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_embo_23_11_2269_s_240	15141169	( Figures 3,  5, and  7), and that IE2 deletion mutants (aa 136 579 and 169 579) lacking the minimal N-terminal  HAT inhibitory domain failed to repress the  in vivo DNA binding of p53 and local histone acetylation ( Figures 1C,  5,  7E, F,  8, and  9).	bind
5125	2	2143	7	10	NULL	0	NULL	Histone	GP		undergoes					acetylation	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_11_2269_s_240	15141169	( Figures 3,  5, and  7), and that IE2 deletion mutants (aa 136 579 and 169 579) lacking the minimal N-terminal  HAT inhibitory domain failed to repress the  in vivo DNA binding of p53 and local histone acetylation ( Figures 1C,  5,  7E, F,  8, and  9).	bind
5126	3	2143	7	10	NULL	0	NULL	IE2	GP	deletion mutants 	lacks			aa 136 579;;169 579					N-terminal HAT inhibitory domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_11_2269_s_240	15141169	( Figures 3,  5, and  7), and that IE2 deletion mutants (aa 136 579 and 169 579) lacking the minimal N-terminal  HAT inhibitory domain failed to repress the  in vivo DNA binding of p53 and local histone acetylation ( Figures 1C,  5,  7E, F,  8, and  9).	bind
5127	4	2143	7	10	NULL	0	NULL	statement 3	Process		does not repress					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_11_2269_s_240	15141169	( Figures 3,  5, and  7), and that IE2 deletion mutants (aa 136 579 and 169 579) lacking the minimal N-terminal  HAT inhibitory domain failed to repress the  in vivo DNA binding of p53 and local histone acetylation ( Figures 1C,  5,  7E, F,  8, and  9).	bind
5128	5	2143	7	10	NULL	0	NULL	statement 3	Process		does not repress					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_11_2269_s_240	15141169	( Figures 3,  5, and  7), and that IE2 deletion mutants (aa 136 579 and 169 579) lacking the minimal N-terminal  HAT inhibitory domain failed to repress the  in vivo DNA binding of p53 and local histone acetylation ( Figures 1C,  5,  7E, F,  8, and  9).	bind
3397	1	2144	6	10	NULL	0	NULL	KIF1A	GP		bind			N-terminal motor domain		MT	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1506_s_234	15014437	( Figures 4 and  5) and that disruption of this interaction enhances MT binding of KIF1A mainly through  the N-terminal motor domain ( Figure 6).	bind
5129	1	2144	7	10	NULL	0	NULL	MT 	CellComponent		binds					KIF1A	GP		N-terminal motor domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1506_s_234	15014437	( Figures 4 and  5) and that disruption of this interaction enhances MT binding of KIF1A mainly through  the N-terminal motor domain ( Figure 6).	bind
3398	1	2145	6	10	NULL	0	NULL	CREB	GP		bind					Egr-1	GP			CRE motif in promoter	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1029_s_174	16497989	( Figures 4 and 5  ) indicate that LPA induces binding activities of CREB and SRF to the CRE and SRE motifs in the Egr-1 promoter, suggesting that CRE and the proximal SRE motifs of the Egr-1 promoter possibly contribute to LPA activation of Egr-1 transcription.	bind
3399	2	2145	6	10	NULL	0	NULL	CREB	GP		bind					Egr-1	GP			SRE motif in promoter	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1029_s_174	16497989	( Figures 4 and 5  ) indicate that LPA induces binding activities of CREB and SRF to the CRE and SRE motifs in the Egr-1 promoter, suggesting that CRE and the proximal SRE motifs of the Egr-1 promoter possibly contribute to LPA activation of Egr-1 transcription.	bind
3400	3	2145	6	10	NULL	0	NULL	LPA	Chemical		induces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1029_s_174	16497989	( Figures 4 and 5  ) indicate that LPA induces binding activities of CREB and SRF to the CRE and SRE motifs in the Egr-1 promoter, suggesting that CRE and the proximal SRE motifs of the Egr-1 promoter possibly contribute to LPA activation of Egr-1 transcription.	bind
3401	4	2145	6	10	NULL	0	NULL	LPA	Chemical		induces					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1029_s_174	16497989	( Figures 4 and 5  ) indicate that LPA induces binding activities of CREB and SRF to the CRE and SRE motifs in the Egr-1 promoter, suggesting that CRE and the proximal SRE motifs of the Egr-1 promoter possibly contribute to LPA activation of Egr-1 transcription.	bind
3402	5	2145	6	10	NULL	0	NULL	SRF	GP		bind					Egr-1	GP			CRE motif in promoter	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1029_s_174	16497989	( Figures 4 and 5  ) indicate that LPA induces binding activities of CREB and SRF to the CRE and SRE motifs in the Egr-1 promoter, suggesting that CRE and the proximal SRE motifs of the Egr-1 promoter possibly contribute to LPA activation of Egr-1 transcription.	bind
3403	6	2145	6	10	NULL	0	NULL	SRF	GP		bind					Egr-1	GP			SRE motif in promoter	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1029_s_174	16497989	( Figures 4 and 5  ) indicate that LPA induces binding activities of CREB and SRF to the CRE and SRE motifs in the Egr-1 promoter, suggesting that CRE and the proximal SRE motifs of the Egr-1 promoter possibly contribute to LPA activation of Egr-1 transcription.	bind
3404	7	2145	6	10	NULL	0	NULL	LPA	Chemical		induces					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1029_s_174	16497989	( Figures 4 and 5  ) indicate that LPA induces binding activities of CREB and SRF to the CRE and SRE motifs in the Egr-1 promoter, suggesting that CRE and the proximal SRE motifs of the Egr-1 promoter possibly contribute to LPA activation of Egr-1 transcription.	bind
3405	8	2145	6	10	NULL	0	NULL	LPA	Chemical		induces					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1029_s_174	16497989	( Figures 4 and 5  ) indicate that LPA induces binding activities of CREB and SRF to the CRE and SRE motifs in the Egr-1 promoter, suggesting that CRE and the proximal SRE motifs of the Egr-1 promoter possibly contribute to LPA activation of Egr-1 transcription.	bind
3406	9	2145	6	10	NULL	0	NULL	LPA	Chemical		activates					Egr-1	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1029_s_174	16497989	( Figures 4 and 5  ) indicate that LPA induces binding activities of CREB and SRF to the CRE and SRE motifs in the Egr-1 promoter, suggesting that CRE and the proximal SRE motifs of the Egr-1 promoter possibly contribute to LPA activation of Egr-1 transcription.	bind
3407	10	2145	6	10	NULL	0	NULL	Egr-1	GP		contribute		possibly		CRE motif of promoter	statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1029_s_174	16497989	( Figures 4 and 5  ) indicate that LPA induces binding activities of CREB and SRF to the CRE and SRE motifs in the Egr-1 promoter, suggesting that CRE and the proximal SRE motifs of the Egr-1 promoter possibly contribute to LPA activation of Egr-1 transcription.	bind
3408	11	2145	6	10	NULL	0	NULL	Egr-1	GP		contribute		possibly		SRE motif of promoter	statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1029_s_174	16497989	( Figures 4 and 5  ) indicate that LPA induces binding activities of CREB and SRF to the CRE and SRE motifs in the Egr-1 promoter, suggesting that CRE and the proximal SRE motifs of the Egr-1 promoter possibly contribute to LPA activation of Egr-1 transcription.	bind
5130	1	2145	7	10	NULL	0	NULL	CREB	GP		binds					Egr-1	GP			CRE motifs in the promoter	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1029_s_174	16497989	( Figures 4 and 5  ) indicate that LPA induces binding activities of CREB and SRF to the CRE and SRE motifs in the Egr-1 promoter, suggesting that CRE and the proximal SRE motifs of the Egr-1 promoter possibly contribute to LPA activation of Egr-1 transcription.	bind
5131	2	2145	7	10	NULL	0	NULL	SRF	GP		binds to					Egr-1	GP			proximal SRE motifs in the promoter of	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1029_s_174	16497989	( Figures 4 and 5  ) indicate that LPA induces binding activities of CREB and SRF to the CRE and SRE motifs in the Egr-1 promoter, suggesting that CRE and the proximal SRE motifs of the Egr-1 promoter possibly contribute to LPA activation of Egr-1 transcription.	bind
5132	3	2145	7	10	NULL	0	NULL	LPA	Chemical		induces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1029_s_174	16497989	( Figures 4 and 5  ) indicate that LPA induces binding activities of CREB and SRF to the CRE and SRE motifs in the Egr-1 promoter, suggesting that CRE and the proximal SRE motifs of the Egr-1 promoter possibly contribute to LPA activation of Egr-1 transcription.	bind
5133	4	2145	7	10	NULL	0	NULL	LPA	Chemical		induces					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1029_s_174	16497989	( Figures 4 and 5  ) indicate that LPA induces binding activities of CREB and SRF to the CRE and SRE motifs in the Egr-1 promoter, suggesting that CRE and the proximal SRE motifs of the Egr-1 promoter possibly contribute to LPA activation of Egr-1 transcription.	bind
5134	5	2145	7	10	NULL	0	NULL	LPA	Chemical		activates					Egr-1	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1029_s_174	16497989	( Figures 4 and 5  ) indicate that LPA induces binding activities of CREB and SRF to the CRE and SRE motifs in the Egr-1 promoter, suggesting that CRE and the proximal SRE motifs of the Egr-1 promoter possibly contribute to LPA activation of Egr-1 transcription.	bind
5135	6	2145	7	10	NULL	0	NULL	Egr-1	GP		contributes		possibly		CRE motifs in the promoter of	statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1029_s_174	16497989	( Figures 4 and 5  ) indicate that LPA induces binding activities of CREB and SRF to the CRE and SRE motifs in the Egr-1 promoter, suggesting that CRE and the proximal SRE motifs of the Egr-1 promoter possibly contribute to LPA activation of Egr-1 transcription.	bind
5136	7	2145	7	10	NULL	0	NULL	Egr-1	GP		contributes		possibly		proximal SRE motifs in the promoter of	statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1029_s_174	16497989	( Figures 4 and 5  ) indicate that LPA induces binding activities of CREB and SRF to the CRE and SRE motifs in the Egr-1 promoter, suggesting that CRE and the proximal SRE motifs of the Egr-1 promoter possibly contribute to LPA activation of Egr-1 transcription.	bind
46284	8	2145	7	10	NULL	0	NULL	CREB	GP		bind					Egr-1	GP			proximal SRE motifs in the promoter of	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1029_s_174	16497989	( Figures 4 and 5  ) indicate that LPA induces binding activities of CREB and SRF to the CRE and SRE motifs in the Egr-1 promoter, suggesting that CRE and the proximal SRE motifs of the Egr-1 promoter possibly contribute to LPA activation of Egr-1 transcription.	bind
46285	9	2145	7	10	NULL	0	NULL	SRF	GP		bind					Egr-1	GP			CRE motifs in the promoter	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1029_s_174	16497989	( Figures 4 and 5  ) indicate that LPA induces binding activities of CREB and SRF to the CRE and SRE motifs in the Egr-1 promoter, suggesting that CRE and the proximal SRE motifs of the Egr-1 promoter possibly contribute to LPA activation of Egr-1 transcription.	bind
46286	10	2145	7	10	NULL	0	NULL	LPA	Chemical		induce					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1029_s_174	16497989	( Figures 4 and 5  ) indicate that LPA induces binding activities of CREB and SRF to the CRE and SRE motifs in the Egr-1 promoter, suggesting that CRE and the proximal SRE motifs of the Egr-1 promoter possibly contribute to LPA activation of Egr-1 transcription.	bind
46287	11	2145	7	10	NULL	0	NULL	LPA	Chemical		induce					statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1029_s_174	16497989	( Figures 4 and 5  ) indicate that LPA induces binding activities of CREB and SRF to the CRE and SRE motifs in the Egr-1 promoter, suggesting that CRE and the proximal SRE motifs of the Egr-1 promoter possibly contribute to LPA activation of Egr-1 transcription.	bind
3409	1	2146	6	10	NULL	0	NULL	Ca+2	Chemical		bind					myofilaments	CellComponent		TnT-I79N		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_4_428_s_223	12600890	( Figures 6 and 8) with no change in L-type Ca2+ current ( Figure 5B) and SR Ca2+ content ( Figure 8F) suggests that initially more Ca2+ is bound to TnT-I79N containing myofilaments, but later on, as the muscle starts to relax, the additional Ca2+ that comes off the myofilaments produces the slower decay of Ca2+ transients.	bind
5137	1	2146	7	10	NULL	0	NULL	Ca2+	Chemical		binds					myofilaments	CellComponent		TnT-I79N		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_4_428_s_223	12600890	( Figures 6 and 8) with no change in L-type Ca2+ current ( Figure 5B) and SR Ca2+ content ( Figure 8F) suggests that initially more Ca2+ is bound to TnT-I79N containing myofilaments, but later on, as the muscle starts to relax, the additional Ca2+ that comes off the myofilaments produces the slower decay of Ca2+ transients.	bind
3651	1	2148	6	10	NULL	0	NULL	IgG	GP		bind					anchoring fibrils	CellComponent				NULL	lamina densa of the dermoepidermal junction	NULL	NULL	NULL	NULL	gw70_jclininvest_116_5_1159_s_30	16670756	( G -  I) Epidermolysis bullosa acquisita is associated with IgG (and sometimes IgA) binding  to the anchoring fibrils underneath the lamina densa of the dermoepidermal junction  ( G), resulting in a subepidermal loss of adhesion ( H) and tense blisters with a tendency toward scarring and milia formation	bind
3652	2	2148	6	10	NULL	0	NULL	statement 1	Process		leads to 					adhesion	Process	subepidermal loss of			NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_5_1159_s_30	16670756	( G -  I) Epidermolysis bullosa acquisita is associated with IgG (and sometimes IgA) binding  to the anchoring fibrils underneath the lamina densa of the dermoepidermal junction  ( G), resulting in a subepidermal loss of adhesion ( H) and tense blisters with a tendency toward scarring and milia formation	bind
3800	3	2148	6	10	NULL	0	NULL	IgA	GP		bind		sometimes			anchoring fibrils	CellComponent				NULL	lamina densa of the dermoepidermal junction	NULL	NULL	NULL	NULL	gw70_jclininvest_116_5_1159_s_30	16670756	( G -  I) Epidermolysis bullosa acquisita is associated with IgG (and sometimes IgA) binding  to the anchoring fibrils underneath the lamina densa of the dermoepidermal junction  ( G), resulting in a subepidermal loss of adhesion ( H) and tense blisters with a tendency toward scarring and milia formation	bind
3801	4	2148	6	10	NULL	0	NULL	Epidermolysis bullosa acquisita			is associated with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_5_1159_s_30	16670756	( G -  I) Epidermolysis bullosa acquisita is associated with IgG (and sometimes IgA) binding  to the anchoring fibrils underneath the lamina densa of the dermoepidermal junction  ( G), resulting in a subepidermal loss of adhesion ( H) and tense blisters with a tendency toward scarring and milia formation	bind
3802	5	2148	6	10	NULL	0	NULL	Epidermolysis bullosa acquisita			is associated with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_5_1159_s_30	16670756	( G -  I) Epidermolysis bullosa acquisita is associated with IgG (and sometimes IgA) binding  to the anchoring fibrils underneath the lamina densa of the dermoepidermal junction  ( G), resulting in a subepidermal loss of adhesion ( H) and tense blisters with a tendency toward scarring and milia formation	bind
5138	1	2148	7	10	NULL	0	NULL	 IgG 	GP		binds					anchoring fibrils	CellComponent				NULL	underneath the lamina densa of the dermoepidermal junction	NULL	NULL	NULL	NULL	gw70_jclininvest_116_5_1159_s_30	16670756	( G -  I) Epidermolysis bullosa acquisita is associated with IgG (and sometimes IgA) binding  to the anchoring fibrils underneath the lamina densa of the dermoepidermal junction  ( G), resulting in a subepidermal loss of adhesion ( H) and tense blisters with a tendency toward scarring and milia formation	bind
5139	2	2148	7	10	NULL	0	NULL	IgA	GP		binds					anchoring fibrils	CellComponent				NULL	underneath the lamina densa of the dermoepidermal junction	NULL	NULL	NULL	NULL	gw70_jclininvest_116_5_1159_s_30	16670756	( G -  I) Epidermolysis bullosa acquisita is associated with IgG (and sometimes IgA) binding  to the anchoring fibrils underneath the lamina densa of the dermoepidermal junction  ( G), resulting in a subepidermal loss of adhesion ( H) and tense blisters with a tendency toward scarring and milia formation	bind
5140	3	2148	7	10	NULL	0	NULL	Epidermolysis bullosa acquisita			is associated with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_5_1159_s_30	16670756	( G -  I) Epidermolysis bullosa acquisita is associated with IgG (and sometimes IgA) binding  to the anchoring fibrils underneath the lamina densa of the dermoepidermal junction  ( G), resulting in a subepidermal loss of adhesion ( H) and tense blisters with a tendency toward scarring and milia formation	bind
5141	4	2148	7	10	NULL	0	NULL	Epidermolysis bullosa acquisita			is associated with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_5_1159_s_30	16670756	( G -  I) Epidermolysis bullosa acquisita is associated with IgG (and sometimes IgA) binding  to the anchoring fibrils underneath the lamina densa of the dermoepidermal junction  ( G), resulting in a subepidermal loss of adhesion ( H) and tense blisters with a tendency toward scarring and milia formation	bind
5142	5	2148	7	10	NULL	0	NULL	statement 1	Process		results in					adhesion	Process	 subepidermal loss of			NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_5_1159_s_30	16670756	( G -  I) Epidermolysis bullosa acquisita is associated with IgG (and sometimes IgA) binding  to the anchoring fibrils underneath the lamina densa of the dermoepidermal junction  ( G), resulting in a subepidermal loss of adhesion ( H) and tense blisters with a tendency toward scarring and milia formation	bind
5143	6	2148	7	10	NULL	0	NULL	statement 2	Process		results in					adhesion	Process	subepidermal loss of			NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_5_1159_s_30	16670756	( G -  I) Epidermolysis bullosa acquisita is associated with IgG (and sometimes IgA) binding  to the anchoring fibrils underneath the lamina densa of the dermoepidermal junction  ( G), resulting in a subepidermal loss of adhesion ( H) and tense blisters with a tendency toward scarring and milia formation	bind
6251	7	2148	7	10	NULL	0	NULL	statement 1	Process		results in					tense blisters	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_5_1159_s_30	16670756	( G -  I) Epidermolysis bullosa acquisita is associated with IgG (and sometimes IgA) binding  to the anchoring fibrils underneath the lamina densa of the dermoepidermal junction  ( G), resulting in a subepidermal loss of adhesion ( H) and tense blisters with a tendency toward scarring and milia formation	bind
6252	9	2148	7	10	NULL	0	NULL	tense blisters			has tendency toward					scarring	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_5_1159_s_30	16670756	( G -  I) Epidermolysis bullosa acquisita is associated with IgG (and sometimes IgA) binding  to the anchoring fibrils underneath the lamina densa of the dermoepidermal junction  ( G), resulting in a subepidermal loss of adhesion ( H) and tense blisters with a tendency toward scarring and milia formation	bind
46288	10	2148	7	10	NULL	0	NULL	tense blisters			has tendency toward					milia formation	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_5_1159_s_30	16670756	( G -  I) Epidermolysis bullosa acquisita is associated with IgG (and sometimes IgA) binding  to the anchoring fibrils underneath the lamina densa of the dermoepidermal junction  ( G), resulting in a subepidermal loss of adhesion ( H) and tense blisters with a tendency toward scarring and milia formation	bind
46289	8	2148	7	10	NULL	0	NULL	statement 2	Process		results in					tense blisters	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_5_1159_s_30	16670756	( G -  I) Epidermolysis bullosa acquisita is associated with IgG (and sometimes IgA) binding  to the anchoring fibrils underneath the lamina densa of the dermoepidermal junction  ( G), resulting in a subepidermal loss of adhesion ( H) and tense blisters with a tendency toward scarring and milia formation	bind
3410	1	2149	6	10	NULL	0	NULL	Akt	GP		bind					Ebp1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_10_2083_s_157	16642037	( G) Akt binds Ebp1 in an NGF-dependent manner.	bind
3411	2	2149	6	10	NULL	0	NULL	statement 1	Process		dependent on					NGF	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_10_2083_s_157	16642037	( G) Akt binds Ebp1 in an NGF-dependent manner.	bind
5144	1	2149	7	10	NULL	0	NULL	Akt	GP		binds					Ebp1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_10_2083_s_157	16642037	( G) Akt binds Ebp1 in an NGF-dependent manner.	bind
5145	2	2149	7	10	NULL	0	NULL	statement 1	Process		is dependent on					NGF	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_10_2083_s_157	16642037	( G) Akt binds Ebp1 in an NGF-dependent manner.	bind
3412	1	2150	6	10	NULL	0	NULL	AP-Nogo-66	GP		bind					Fc-MAG	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_297_5584_1190_s_50	12089450	( G) AP-Nogo-66 or AP-NgR bound to Fc-MAG.	bind
3413	2	2150	6	10	NULL	0	NULL	AP-NgR	GP		bind					Fc-MAG	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_297_5584_1190_s_50	12089450	( G) AP-Nogo-66 or AP-NgR bound to Fc-MAG.	bind
4397	3	2150	6	10	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_297_5584_1190_s_50	12089450	( G) AP-Nogo-66 or AP-NgR bound to Fc-MAG.	bind
5146	1	2150	7	10	NULL	0	NULL	 AP-Nogo-66	GP		binds					Fc-MAG	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_297_5584_1190_s_50	12089450	( G) AP-Nogo-66 or AP-NgR bound to Fc-MAG.	bind
5147	2	2150	7	10	NULL	0	NULL	AP-NgR	GP		binds					Fc-MAG	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_297_5584_1190_s_50	12089450	( G) AP-Nogo-66 or AP-NgR bound to Fc-MAG.	bind
51552	3	2150	7	10	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_297_5584_1190_s_50	12089450	( G) AP-Nogo-66 or AP-NgR bound to Fc-MAG.	bind
3414	1	2151	6	10	NULL	0	NULL	PAIRED DNA	NucleicAcid		bind									100 bp so probe	NULL		NULL	NULL	NULL	NULL	gw60_embo_20_4_802_s_187	11179224	( G) Bacterially synthesized ANTP HD inhibits PAIRED DNA binding to the 100 bp  so probe ( Niimi  et al., 1999).	bind
3415	2	2151	6	10	NULL	0	NULL	ANTP	GP	bacterially synthesized	inhibits			HD		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_4_802_s_187	11179224	( G) Bacterially synthesized ANTP HD inhibits PAIRED DNA binding to the 100 bp  so probe ( Niimi  et al., 1999).	bind
5148	1	2151	7	10	NULL	0	NULL	PAIRED DNA	NucleicAcid		binds									100 bp	NULL		NULL	NULL	NULL	NULL	gw60_embo_20_4_802_s_187	11179224	( G) Bacterially synthesized ANTP HD inhibits PAIRED DNA binding to the 100 bp  so probe ( Niimi  et al., 1999).	bind
5149	2	2151	7	10	NULL	0	NULL	ANTP	GP	Bacterially synthesized	inhibits			HD		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_4_802_s_187	11179224	( G) Bacterially synthesized ANTP HD inhibits PAIRED DNA binding to the 100 bp  so probe ( Niimi  et al., 1999).	bind
3416	1	2152	6	10	NULL	0	NULL	LyP-1	GP		bind					MDA-MB-435 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_20_12617_s_78	12235356	( g) Binding of LyP-1 qdots to MDA-MB-435 cells.	bind
5150	1	2152	7	10	NULL	0	NULL	LyP-1	GP		binds to					MDA-MB-435 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_20_12617_s_78	12235356	( g) Binding of LyP-1 qdots to MDA-MB-435 cells.	bind
3417	1	2153	6	10	NULL	0	NULL	Myc	GP		bind					Miz-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_2_336_s_169	15616584	( G) Corepression of  p21Cip1 by Myc and Dnmt3a requires binding of Myc to Miz-1.	bind
3418	2	2153	6	10	NULL	0	NULL	Myc	GP		corepresses					p21Cip1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_2_336_s_169	15616584	( G) Corepression of  p21Cip1 by Myc and Dnmt3a requires binding of Myc to Miz-1.	bind
3419	3	2153	6	10	NULL	0	NULL	Dnmt3a	GP		corepresses					p21Cip1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_2_336_s_169	15616584	( G) Corepression of  p21Cip1 by Myc and Dnmt3a requires binding of Myc to Miz-1.	bind
3420	4	2153	6	10	NULL	0	NULL	statement 2	Process		requires					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_2_336_s_169	15616584	( G) Corepression of  p21Cip1 by Myc and Dnmt3a requires binding of Myc to Miz-1.	bind
3421	5	2153	6	10	NULL	0	NULL	statement 3	Process		requires					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_2_336_s_169	15616584	( G) Corepression of  p21Cip1 by Myc and Dnmt3a requires binding of Myc to Miz-1.	bind
5151	1	2153	7	10	NULL	0	NULL	Myc	GP		binds					Miz-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_2_336_s_169	15616584	( G) Corepression of  p21Cip1 by Myc and Dnmt3a requires binding of Myc to Miz-1.	bind
5152	2	2153	7	10	NULL	0	NULL	Myc	GP		corepress					p21Cip1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_2_336_s_169	15616584	( G) Corepression of  p21Cip1 by Myc and Dnmt3a requires binding of Myc to Miz-1.	bind
5153	3	2153	7	10	NULL	0	NULL	Dnmt3a	GP		corepress					p21Cip1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_2_336_s_169	15616584	( G) Corepression of  p21Cip1 by Myc and Dnmt3a requires binding of Myc to Miz-1.	bind
5154	4	2153	7	10	NULL	0	NULL	statement 2	Process		requires					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_2_336_s_169	15616584	( G) Corepression of  p21Cip1 by Myc and Dnmt3a requires binding of Myc to Miz-1.	bind
5155	5	2153	7	10	NULL	0	NULL	statement 3	Process		requires					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_2_336_s_169	15616584	( G) Corepression of  p21Cip1 by Myc and Dnmt3a requires binding of Myc to Miz-1.	bind
3422	1	2155	6	10	NULL	0	NULL	RAD50	GP	human	bind			NH2-terminus		BRCA1	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_285_5428_747_s_40	10426999	( G) NH2-terminus of hRad50 binds BRCA1 in a yeast two-hybrid assay.	bind
5156	1	2155	7	10	NULL	0	NULL	hRad50	GP		binds			NH2-terminus		BRCA1	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_285_5428_747_s_40	10426999	( G) NH2-terminus of hRad50 binds BRCA1 in a yeast two-hybrid assay.	bind
3423	1	2156	6	10	NULL	0	NULL	CaBP1	GP		bind					Ins P3R-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_11_7711_s_163	12032348	( G) Quantitative analysis of competition for CaBP1 binding to Ins P3R-3 by s-CaBP1 with data normalized to binding in the absence of added s-CaBP1.	bind
3424	2	2156	6	10	NULL	0	NULL	s-CaBP1	GP		bind					Ins P3R-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_11_7711_s_163	12032348	( G) Quantitative analysis of competition for CaBP1 binding to Ins P3R-3 by s-CaBP1 with data normalized to binding in the absence of added s-CaBP1.	bind
3425	3	2156	6	10	NULL	0	NULL	statement 1	Process		competes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_11_7711_s_163	12032348	( G) Quantitative analysis of competition for CaBP1 binding to Ins P3R-3 by s-CaBP1 with data normalized to binding in the absence of added s-CaBP1.	bind
5157	1	2156	7	10	NULL	0	NULL	CaBP1	GP		binds					Ins P3R-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_11_7711_s_163	12032348	( G) Quantitative analysis of competition for CaBP1 binding to Ins P3R-3 by s-CaBP1 with data normalized to binding in the absence of added s-CaBP1.	bind
5158	2	2156	7	10	NULL	0	NULL	 s-CaBP1	GP		binds					Ins P3R-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_11_7711_s_163	12032348	( G) Quantitative analysis of competition for CaBP1 binding to Ins P3R-3 by s-CaBP1 with data normalized to binding in the absence of added s-CaBP1.	bind
5159	3	2156	7	10	NULL	0	NULL	statement 2	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_11_7711_s_163	12032348	( G) Quantitative analysis of competition for CaBP1 binding to Ins P3R-3 by s-CaBP1 with data normalized to binding in the absence of added s-CaBP1.	bind
3426	1	2157	6	10	NULL	0	NULL	MukF	GP	tagged	bind			331 440		MukB	GP		ATPase domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_11_1921_s_143	15902272	( G) Tagged MukF(331 440) binds the ATPase domain of MukB.	bind
5160	1	2157	7	10	NULL	0	NULL	MukF	GP	Tagged	binds			331 440		MukB	GP		ATPase domain of		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_11_1921_s_143	15902272	( G) Tagged MukF(331 440) binds the ATPase domain of MukB.	bind
3427	1	2158	6	10	NULL	0	NULL	Triol	GP		bind		directly			PXR	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_3_833_s_78	12569201	( g) Triol binds directly to PXR.	bind
5161	1	2158	7	10	NULL	0	NULL	Triol 	GP		binds		directly			PXR	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_3_833_s_78	12569201	( g) Triol binds directly to PXR.	bind
3428	1	2159	6	10	NULL	0	NULL	GST-Six3	GP	bacteria expressed	bind		strongly			Wnt1	GP			element I of promoter	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_3_368_s_140	12569128	( G``) A magnification of the electroporated embryo shown in  G. ( H) EMSA assay shows that bacteria-expressed GST-Six3 fusion protein binds to the  Wnt1 promoter elements I and II (lanes  3,8) strongly, very weakly to element III (lane  13), and not at all to element IV (data not shown).	bind
3429	2	2159	6	10	NULL	0	NULL	GST-Six3	GP	bacteria expressed	bind		strongly			Wnt1	GP			element II of promoter	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_3_368_s_140	12569128	( G``) A magnification of the electroporated embryo shown in  G. ( H) EMSA assay shows that bacteria-expressed GST-Six3 fusion protein binds to the  Wnt1 promoter elements I and II (lanes  3,8) strongly, very weakly to element III (lane  13), and not at all to element IV (data not shown).	bind
3430	3	2159	6	10	NULL	0	NULL	GST-Six3	GP	bacteria expressed	bind		weakly			Wnt1	GP			element III of promoter	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_3_368_s_140	12569128	( G``) A magnification of the electroporated embryo shown in  G. ( H) EMSA assay shows that bacteria-expressed GST-Six3 fusion protein binds to the  Wnt1 promoter elements I and II (lanes  3,8) strongly, very weakly to element III (lane  13), and not at all to element IV (data not shown).	bind
3431	4	2159	6	10	NULL	0	NULL	GST-Six3	GP		does not bind					Wnt1	GP			element IV of promoter	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_3_368_s_140	12569128	( G``) A magnification of the electroporated embryo shown in  G. ( H) EMSA assay shows that bacteria-expressed GST-Six3 fusion protein binds to the  Wnt1 promoter elements I and II (lanes  3,8) strongly, very weakly to element III (lane  13), and not at all to element IV (data not shown).	bind
45957	5	2159	6	10	NULL	0	NULL	GST-Six3	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_3_368_s_140	12569128	( G``) A magnification of the electroporated embryo shown in  G. ( H) EMSA assay shows that bacteria-expressed GST-Six3 fusion protein binds to the  Wnt1 promoter elements I and II (lanes  3,8) strongly, very weakly to element III (lane  13), and not at all to element IV (data not shown).	bind
5162	1	2159	7	10	NULL	0	NULL	GST-Six3	GP	bacteria-expressed	binds to		strongly			Wnt1	GP			promoter elements I	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_3_368_s_140	12569128	( G``) A magnification of the electroporated embryo shown in  G. ( H) EMSA assay shows that bacteria-expressed GST-Six3 fusion protein binds to the  Wnt1 promoter elements I and II (lanes  3,8) strongly, very weakly to element III (lane  13), and not at all to element IV (data not shown).	bind
5163	2	2159	7	10	NULL	0	NULL	GST-Six3	GP	bacteria-expressed	binds to		strongly			Wnt1	GP			promoter elements II	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_3_368_s_140	12569128	( G``) A magnification of the electroporated embryo shown in  G. ( H) EMSA assay shows that bacteria-expressed GST-Six3 fusion protein binds to the  Wnt1 promoter elements I and II (lanes  3,8) strongly, very weakly to element III (lane  13), and not at all to element IV (data not shown).	bind
5164	3	2159	7	10	NULL	0	NULL	GST-Six3	GP	bacteria-expressed	binds to		very weakly			Wnt1	GP			promoter elements III	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_3_368_s_140	12569128	( G``) A magnification of the electroporated embryo shown in  G. ( H) EMSA assay shows that bacteria-expressed GST-Six3 fusion protein binds to the  Wnt1 promoter elements I and II (lanes  3,8) strongly, very weakly to element III (lane  13), and not at all to element IV (data not shown).	bind
5165	4	2159	7	10	NULL	0	NULL	GST-Six3	GP	bacteria-expressed	does not bind					Wnt1	GP			promoter elements IV	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_3_368_s_140	12569128	( G``) A magnification of the electroporated embryo shown in  G. ( H) EMSA assay shows that bacteria-expressed GST-Six3 fusion protein binds to the  Wnt1 promoter elements I and II (lanes  3,8) strongly, very weakly to element III (lane  13), and not at all to element IV (data not shown).	bind
45956	5	2159	7	10	NULL	0	NULL	GST-Six3	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_3_368_s_140	12569128	( G``) A magnification of the electroporated embryo shown in  G. ( H) EMSA assay shows that bacteria-expressed GST-Six3 fusion protein binds to the  Wnt1 promoter elements I and II (lanes  3,8) strongly, very weakly to element III (lane  13), and not at all to element IV (data not shown).	bind
3432	1	2160	6	10	NULL	0	NULL	ATX1	GP	cellular	bind					PI5P	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_15_6049_s_132	16585509	( H and  I) Cellular ATX1 binds PI5P.	bind
5166	1	2160	7	10	NULL	0	NULL	ATX1	GP	cellular	binds					PI5P	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_15_6049_s_132	16585509	( H and  I) Cellular ATX1 binds PI5P.	bind
3433	1	2161	6	10	NULL	0	NULL	LyP-1	GP		does not bind					LE cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_20_12617_s_79	12235356	( h and  i) GFE qdots do not recognize the MDA-MB-435 cells ( h) and LyP-1 qdots do not bind to the LE cells ( i).	bind
3434	2	2161	6	10	NULL	0	NULL	GFE	GP		does not recognize					MDA-MB-435 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_20_12617_s_79	12235356	( h and  i) GFE qdots do not recognize the MDA-MB-435 cells ( h) and LyP-1 qdots do not bind to the LE cells ( i).	bind
5167	1	2161	7	10	NULL	0	NULL	GFE 	GP		do not recognize					MDA-MB-435 cells 	Cell				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_20_12617_s_79	12235356	( h and  i) GFE qdots do not recognize the MDA-MB-435 cells ( h) and LyP-1 qdots do not bind to the LE cells ( i).	bind
5168	2	2161	7	10	NULL	0	NULL	 LyP-1	GP		does not bind					LE cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_20_12617_s_79	12235356	( h and  i) GFE qdots do not recognize the MDA-MB-435 cells ( h) and LyP-1 qdots do not bind to the LE cells ( i).	bind
3435	1	2162	6	10	NULL	0	NULL	M1 RNA	NucleicAcid		bind					Rpp29	GP		KH		NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_16_5120_s_282	16155184	( H) Binding of M1 RNA by the indicated concentrations of Rpp29KH (lanes 2 - 4) or Rpp29K179N  (lanes 5 - 7).	bind
3436	2	2162	6	10	NULL	0	NULL	M1 RNA	NucleicAcid		bind					Rpp29	GP		K179N		NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_16_5120_s_282	16155184	( H) Binding of M1 RNA by the indicated concentrations of Rpp29KH (lanes 2 - 4) or Rpp29K179N  (lanes 5 - 7).	bind
5169	1	2162	7	10	NULL	0	NULL	Rpp29	GP		binds			KH		M1RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_16_5120_s_282	16155184	( H) Binding of M1 RNA by the indicated concentrations of Rpp29KH (lanes 2 - 4) or Rpp29K179N  (lanes 5 - 7).	bind
5170	2	2162	7	10	NULL	0	NULL	Rpp29	GP		binds			K179N		M1RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_16_5120_s_282	16155184	( H) Binding of M1 RNA by the indicated concentrations of Rpp29KH (lanes 2 - 4) or Rpp29K179N  (lanes 5 - 7).	bind
3437	1	2163	6	10	NULL	0	NULL	E2F	GP		bind					hTERT	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_31_11328_s_137	15263087	( H) Changes in the binding of E2F and pocket proteins to the hTERT promoter during the  cell cycle.	bind
3438	2	2163	6	10	NULL	0	NULL	pocket proteins	GP		bind					hTERT	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_31_11328_s_137	15263087	( H) Changes in the binding of E2F and pocket proteins to the hTERT promoter during the  cell cycle.	bind
5171	1	2163	7	10	NULL	0	NULL	E2F	GP		binds					hTERT	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_31_11328_s_137	15263087	( H) Changes in the binding of E2F and pocket proteins to the hTERT promoter during the  cell cycle.	bind
5172	2	2163	7	10	NULL	0	NULL	pocket proteins	GP		binds					hTERT	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_31_11328_s_137	15263087	( H) Changes in the binding of E2F and pocket proteins to the hTERT promoter during the  cell cycle.	bind
3439	1	2164	6	10	NULL	0	NULL	CFTR	GP		bind					EBP50	GP				NULL	calu-3 cells 	NULL	NULL	NULL	NULL	gw70_pnas_100_1_342_s_185	12502786	( H) Coimmunoprecipitation of CFTR and EBP50 from calu-3 cells treated with or without  cpt-cAMP mixture for 10 min at 37 degrees C. cpt-cAMP treatment diminishes EBP50  binding during coimmunoprecipitation.	bind
3441	2	2164	6	10	NULL	0	NULL	cpt-cAMP	Chemical	treatment of	diminishes					statement 1	Process				NULL	calu-3 cells 	NULL	NULL	NULL	NULL	gw70_pnas_100_1_342_s_185	12502786	( H) Coimmunoprecipitation of CFTR and EBP50 from calu-3 cells treated with or without  cpt-cAMP mixture for 10 min at 37 degrees C. cpt-cAMP treatment diminishes EBP50  binding during coimmunoprecipitation.	bind
6253	1	2164	7	10	NULL	0	NULL	CFTR	GP		binds					EBP50	GP				NULL	calu-3 cells	NULL	NULL	NULL	NULL	gw70_pnas_100_1_342_s_185	12502786	( H) Coimmunoprecipitation of CFTR and EBP50 from calu-3 cells treated with or without  cpt-cAMP mixture for 10 min at 37 degrees C. cpt-cAMP treatment diminishes EBP50  binding during coimmunoprecipitation.	bind
6254	2	2164	7	10	NULL	0	NULL	cpt-cAMP	Chemical	treatment	diminishes					statement 1	Process				NULL	calu-3 cells 	NULL	NULL	NULL	NULL	gw70_pnas_100_1_342_s_185	12502786	( H) Coimmunoprecipitation of CFTR and EBP50 from calu-3 cells treated with or without  cpt-cAMP mixture for 10 min at 37 degrees C. cpt-cAMP treatment diminishes EBP50  binding during coimmunoprecipitation.	bind
3448	1	2168	6	10	NULL	0	NULL	Basonuclin	GP		bind									dyad sequence within BBS1	NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_17_9628_s_203	10449744	( i) Basonuclin binds to two dyad sequences, one completely within BBS1 and the other divided between BBS1 and BBS2.	bind
3449	2	2168	6	10	NULL	0	NULL	Basonuclin	GP		bind									dyad sequence between BBS1 and BBS2	NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_17_9628_s_203	10449744	( i) Basonuclin binds to two dyad sequences, one completely within BBS1 and the other divided between BBS1 and BBS2.	bind
5173	1	2168	7	10	NULL	0	NULL	Basonuclin	GP		binds									dyad sequence within BBS1	NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_17_9628_s_203	10449744	( i) Basonuclin binds to two dyad sequences, one completely within BBS1 and the other divided between BBS1 and BBS2.	bind
5174	2	2168	7	10	NULL	0	NULL	Basonuclin	GP		binds									dyad sequence between BBS1 and BBS2	NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_17_9628_s_203	10449744	( i) Basonuclin binds to two dyad sequences, one completely within BBS1 and the other divided between BBS1 and BBS2.	bind
3450	1	2170	6	10	NULL	0	NULL	NPC1	GP		bind		low affinity			cholesterol	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_34_12473_s_231	15314240	( i) NPC1 binds to cholesterol as its substrate and transports it at the late endosomal membrane; this possibility would be consistent with the current finding that NPC1 binds to cholesterol with low affinity.	bind
3452	2	2170	6	10	NULL	0	NULL	cholesterol	Chemical		is transported to					late endosomal membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_34_12473_s_231	15314240	( i) NPC1 binds to cholesterol as its substrate and transports it at the late endosomal membrane; this possibility would be consistent with the current finding that NPC1 binds to cholesterol with low affinity.	bind
3453	3	2170	6	10	NULL	0	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_34_12473_s_231	15314240	( i) NPC1 binds to cholesterol as its substrate and transports it at the late endosomal membrane; this possibility would be consistent with the current finding that NPC1 binds to cholesterol with low affinity.	bind
5175	1	2170	7	10	NULL	0	NULL	NPC1	GP		binds to		low affinity			cholesterol	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_34_12473_s_231	15314240	( i) NPC1 binds to cholesterol as its substrate and transports it at the late endosomal membrane; this possibility would be consistent with the current finding that NPC1 binds to cholesterol with low affinity.	bind
5176	2	2170	7	10	NULL	0	NULL	cholesterol	Chemical		is transported to					late endosomal membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_34_12473_s_231	15314240	( i) NPC1 binds to cholesterol as its substrate and transports it at the late endosomal membrane; this possibility would be consistent with the current finding that NPC1 binds to cholesterol with low affinity.	bind
5177	3	2170	7	10	NULL	0	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_34_12473_s_231	15314240	( i) NPC1 binds to cholesterol as its substrate and transports it at the late endosomal membrane; this possibility would be consistent with the current finding that NPC1 binds to cholesterol with low affinity.	bind
3454	1	2171	6	10	NULL	0	NULL	ORC	NucleicAcid		bind					ACS	NucleicAcid	essential			NULL	ARS309 in vitro 	NULL	NULL	NULL	NULL	gw60_pnas_94_20_10786_s_134	9380711	( i) Our  in vitro analysis of  ARS309 indicates that ORC binds to the essential ACS.	bind
5178	1	2171	7	10	NULL	0	NULL	ORC	NucleicAcid		binds					ACS	NucleicAcid	essential			NULL	ARS309 in vitro 	NULL	NULL	NULL	NULL	gw60_pnas_94_20_10786_s_134	9380711	( i) Our  in vitro analysis of  ARS309 indicates that ORC binds to the essential ACS.	bind
3456	1	2172	6	10	NULL	0	NULL	S1	GP		bind					actin	GP	oriented			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_9_6011_s_201	11972024	( i) Spectroscopic studies of the orientation of the LC domain, measured by using paramagnetic ( 19) or fluorescent ( 15) probes, have found that the orientation of the LC domains were similar when S1 or HMM were bound to oriented actin, and both were similar to rigor fibers.	bind
3457	2	2172	6	10	NULL	0	NULL	HMM	GP		bind					actin	GP	oriented			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_9_6011_s_201	11972024	( i) Spectroscopic studies of the orientation of the LC domain, measured by using paramagnetic ( 19) or fluorescent ( 15) probes, have found that the orientation of the LC domains were similar when S1 or HMM were bound to oriented actin, and both were similar to rigor fibers.	bind
5180	1	2172	7	10	NULL	0	NULL	S1	GP		binds					actin	GP	oriented			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_9_6011_s_201	11972024	( i) Spectroscopic studies of the orientation of the LC domain, measured by using paramagnetic ( 19) or fluorescent ( 15) probes, have found that the orientation of the LC domains were similar when S1 or HMM were bound to oriented actin, and both were similar to rigor fibers.	bind
5181	2	2172	7	10	NULL	0	NULL	HMM	GP		binds					actin	GP	oriented			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_9_6011_s_201	11972024	( i) Spectroscopic studies of the orientation of the LC domain, measured by using paramagnetic ( 19) or fluorescent ( 15) probes, have found that the orientation of the LC domains were similar when S1 or HMM were bound to oriented actin, and both were similar to rigor fibers.	bind
3458	1	2173	6	10	NULL	0	NULL	icon	GP		bind					vascular endothelium	Cell	human tumor			NULL	SCID mice	NULL	NULL	NULL	NULL	gw60_pnas_98_21_12180_s_248	11593034	( i) The icon binds to the vascular endothelium of a human tumor in SCID mice, but does not bind to the mouse liver or kidney, and probably not to other normal tissues.	bind
3459	2	2173	6	10	NULL	0	NULL	icon	GP		does not bind					liver	OrganismPart	mouse			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_21_12180_s_248	11593034	( i) The icon binds to the vascular endothelium of a human tumor in SCID mice, but does not bind to the mouse liver or kidney, and probably not to other normal tissues.	bind
3460	3	2173	6	10	NULL	0	NULL	icon	GP		does not bind					kidney	OrganismPart	mouse			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_21_12180_s_248	11593034	( i) The icon binds to the vascular endothelium of a human tumor in SCID mice, but does not bind to the mouse liver or kidney, and probably not to other normal tissues.	bind
3461	4	2173	6	10	NULL	0	NULL	icon	GP		does not bind		probably			tissues	OrganismPart	normal			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_21_12180_s_248	11593034	( i) The icon binds to the vascular endothelium of a human tumor in SCID mice, but does not bind to the mouse liver or kidney, and probably not to other normal tissues.	bind
5182	1	2173	7	10	NULL	0	NULL	 icon	GP		binds to					vascular endothelium	OrganismPart	human tumor			NULL	SCID mice	NULL	NULL	NULL	NULL	gw60_pnas_98_21_12180_s_248	11593034	( i) The icon binds to the vascular endothelium of a human tumor in SCID mice, but does not bind to the mouse liver or kidney, and probably not to other normal tissues.	bind
5183	2	2173	7	10	NULL	0	NULL	icon	GP		does not bind					liver	OrganismPart	mouse			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_21_12180_s_248	11593034	( i) The icon binds to the vascular endothelium of a human tumor in SCID mice, but does not bind to the mouse liver or kidney, and probably not to other normal tissues.	bind
5184	3	2173	7	10	NULL	0	NULL	icon	GP		does not bind					kidney	OrganismPart	mouse			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_21_12180_s_248	11593034	( i) The icon binds to the vascular endothelium of a human tumor in SCID mice, but does not bind to the mouse liver or kidney, and probably not to other normal tissues.	bind
5185	4	2173	7	10	NULL	0	NULL	icon	GP		does not bind		probably			tissues	OrganismPart	normal			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_21_12180_s_248	11593034	( i) The icon binds to the vascular endothelium of a human tumor in SCID mice, but does not bind to the mouse liver or kidney, and probably not to other normal tissues.	bind
3463	1	2174	6	10	NULL	0	NULL	TSG101	GP		bind					p6	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_2_955_s_172	11805336	( i) The reported ability of TSG101 and other E2-like proteins to inhibit or modify the target specificity of ubiquitination ( 29,  45) raises the possibility that binding of TSG101 by p6 could alter the extent to which Gag becomes ubiquitinated.	bind
3464	2	2174	6	10	NULL	0	NULL	statement 1	Process		alters					Gag	GP	ubiquitination of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_2_955_s_172	11805336	( i) The reported ability of TSG101 and other E2-like proteins to inhibit or modify the target specificity of ubiquitination ( 29,  45) raises the possibility that binding of TSG101 by p6 could alter the extent to which Gag becomes ubiquitinated.	bind
46195	3	2174	6	10	NULL	0	NULL	TSG101	GP		inhibit					ubiquitination	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_2_955_s_172	11805336	( i) The reported ability of TSG101 and other E2-like proteins to inhibit or modify the target specificity of ubiquitination ( 29,  45) raises the possibility that binding of TSG101 by p6 could alter the extent to which Gag becomes ubiquitinated.	bind
46197	4	2174	6	10	NULL	0	NULL	TSG101	GP		modify					ubiquitination	Process	target specificity of 			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_2_955_s_172	11805336	( i) The reported ability of TSG101 and other E2-like proteins to inhibit or modify the target specificity of ubiquitination ( 29,  45) raises the possibility that binding of TSG101 by p6 could alter the extent to which Gag becomes ubiquitinated.	bind
46198	5	2174	6	10	NULL	0	NULL	E2-like proteins	GP		inhibit					ubiquitination	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_2_955_s_172	11805336	( i) The reported ability of TSG101 and other E2-like proteins to inhibit or modify the target specificity of ubiquitination ( 29,  45) raises the possibility that binding of TSG101 by p6 could alter the extent to which Gag becomes ubiquitinated.	bind
46199	6	2174	6	10	NULL	0	NULL	E2-like proteins	GP		modify					ubiquitination	Process	target specificity of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_2_955_s_172	11805336	( i) The reported ability of TSG101 and other E2-like proteins to inhibit or modify the target specificity of ubiquitination ( 29,  45) raises the possibility that binding of TSG101 by p6 could alter the extent to which Gag becomes ubiquitinated.	bind
51553	7	2174	6	10	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_2_955_s_172	11805336	( i) The reported ability of TSG101 and other E2-like proteins to inhibit or modify the target specificity of ubiquitination ( 29,  45) raises the possibility that binding of TSG101 by p6 could alter the extent to which Gag becomes ubiquitinated.	bind
51554	8	2174	6	10	NULL	0	NULL	statement 5	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_2_955_s_172	11805336	( i) The reported ability of TSG101 and other E2-like proteins to inhibit or modify the target specificity of ubiquitination ( 29,  45) raises the possibility that binding of TSG101 by p6 could alter the extent to which Gag becomes ubiquitinated.	bind
5186	1	2174	7	10	NULL	0	NULL	 p6	GP		binds					TSG101	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_2_955_s_172	11805336	( i) The reported ability of TSG101 and other E2-like proteins to inhibit or modify the target specificity of ubiquitination ( 29,  45) raises the possibility that binding of TSG101 by p6 could alter the extent to which Gag becomes ubiquitinated.	bind
5188	3	2174	7	10	NULL	0	NULL	statement 1	Process		alters					Gag	GP	ubiquitination of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_2_955_s_172	11805336	( i) The reported ability of TSG101 and other E2-like proteins to inhibit or modify the target specificity of ubiquitination ( 29,  45) raises the possibility that binding of TSG101 by p6 could alter the extent to which Gag becomes ubiquitinated.	bind
5189	4	2174	7	10	NULL	0	NULL	TSG101	GP		inhibits					ubiquitination 	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_2_955_s_172	11805336	( i) The reported ability of TSG101 and other E2-like proteins to inhibit or modify the target specificity of ubiquitination ( 29,  45) raises the possibility that binding of TSG101 by p6 could alter the extent to which Gag becomes ubiquitinated.	bind
5190	5	2174	7	10	NULL	0	NULL	TSG101	GP		modify					ubiquitination	Process	target specificity of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_2_955_s_172	11805336	( i) The reported ability of TSG101 and other E2-like proteins to inhibit or modify the target specificity of ubiquitination ( 29,  45) raises the possibility that binding of TSG101 by p6 could alter the extent to which Gag becomes ubiquitinated.	bind
5191	6	2174	7	10	NULL	0	NULL	E2-like proteins	GP		inhibits					ubiquitination	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_2_955_s_172	11805336	( i) The reported ability of TSG101 and other E2-like proteins to inhibit or modify the target specificity of ubiquitination ( 29,  45) raises the possibility that binding of TSG101 by p6 could alter the extent to which Gag becomes ubiquitinated.	bind
5192	7	2174	7	10	NULL	0	NULL	E2-like proteins	GP		modify					ubiquitination	Process	target specificity of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_2_955_s_172	11805336	( i) The reported ability of TSG101 and other E2-like proteins to inhibit or modify the target specificity of ubiquitination ( 29,  45) raises the possibility that binding of TSG101 by p6 could alter the extent to which Gag becomes ubiquitinated.	bind
46290	8	2174	7	10	NULL	0	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_2_955_s_172	11805336	( i) The reported ability of TSG101 and other E2-like proteins to inhibit or modify the target specificity of ubiquitination ( 29,  45) raises the possibility that binding of TSG101 by p6 could alter the extent to which Gag becomes ubiquitinated.	bind
46291	9	2174	7	10	NULL	0	NULL	statement 6	Process		is an alternative to					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_2_955_s_172	11805336	( i) The reported ability of TSG101 and other E2-like proteins to inhibit or modify the target specificity of ubiquitination ( 29,  45) raises the possibility that binding of TSG101 by p6 could alter the extent to which Gag becomes ubiquitinated.	bind
3465	1	2175	6	10	NULL	0	NULL	tRNAIle	NucleicAcid		bind					IleRS/Val-AMP complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_2_585_s_215	11782529	( i) tRNAIle binds to the IleRS/Val-AMP complex.	bind
5193	1	2175	7	10	NULL	0	NULL	tRNAIle	NucleicAcid		binds to					IleRS/Val-AMP complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_2_585_s_215	11782529	( i) tRNAIle binds to the IleRS/Val-AMP complex.	bind
3466	1	2176	6	10	NULL	0	NULL	IP3	GP		bind					type 2 receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_20_17571_s_204	11875073	( I) whether or not they have IP3 bound, whereas IP3 binding protects type 2 receptors from Ca2+ inhibition.	bind
3467	2	2176	6	10	NULL	0	NULL	Ca2+	Chemical		inhibits					type 2 receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_20_17571_s_204	11875073	( I) whether or not they have IP3 bound, whereas IP3 binding protects type 2 receptors from Ca2+ inhibition.	bind
46200	3	2176	6	10	NULL	0	NULL	statement 1	Process		protects					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_20_17571_s_204	11875073	( I) whether or not they have IP3 bound, whereas IP3 binding protects type 2 receptors from Ca2+ inhibition.	bind
5194	1	2176	7	10	NULL	0	NULL	 IP3	GP		binds					type 2 receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_20_17571_s_204	11875073	( I) whether or not they have IP3 bound, whereas IP3 binding protects type 2 receptors from Ca2+ inhibition.	bind
5195	2	2176	7	10	NULL	0	NULL	Ca2+	Chemical		inhibits					type 2 receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_20_17571_s_204	11875073	( I) whether or not they have IP3 bound, whereas IP3 binding protects type 2 receptors from Ca2+ inhibition.	bind
5196	3	2176	7	10	NULL	0	NULL	statement 1	Process		protects					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_20_17571_s_204	11875073	( I) whether or not they have IP3 bound, whereas IP3 binding protects type 2 receptors from Ca2+ inhibition.	bind
3468	1	2178	6	10	NULL	0	NULL	N-3	Chemical		bind					SW Mb	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1594_2_341_s_147	11904230	( I=800 mM) using decreasing concentrations of divalent SO2-4 with both Mbs, or monovalent Cl- only with HH Mb due to the effect that this anion has on N-3 binding to SW Mb (see  Fig. 2).	bind
5370	1	2178	7	10	NULL	0	NULL	N-3	Chemical		binds					SW Mb	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1594_2_341_s_147	11904230	( I=800 mM) using decreasing concentrations of divalent SO2-4 with both Mbs, or monovalent Cl- only with HH Mb due to the effect that this anion has on N-3 binding to SW Mb (see  Fig. 2).	bind
3469	1	2179	6	10	NULL	0	NULL	GalCer	Chemical		bind					P1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25649_s_178	11940580	( If) as a function of P1 concentration exhibits a sharp transition between P1 concentration of 25 and 50 muM in both raft lipids and PBS environment, indicating that the GalCer* binding affinity to the P1 depends strongly on P1 concentration and, therefore, on P1 secondary structure (see Fig.  2).	bind
3470	2	2179	6	10	NULL	0	NULL	statement 1	Process		depends 		strongly			P1	GP	concentration of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25649_s_178	11940580	( If) as a function of P1 concentration exhibits a sharp transition between P1 concentration of 25 and 50 muM in both raft lipids and PBS environment, indicating that the GalCer* binding affinity to the P1 depends strongly on P1 concentration and, therefore, on P1 secondary structure (see Fig.  2).	bind
3471	3	2179	6	10	NULL	0	NULL	statement 1	Process		depends 					P1	GP	secondary structure of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25649_s_178	11940580	( If) as a function of P1 concentration exhibits a sharp transition between P1 concentration of 25 and 50 muM in both raft lipids and PBS environment, indicating that the GalCer* binding affinity to the P1 depends strongly on P1 concentration and, therefore, on P1 secondary structure (see Fig.  2).	bind
5372	1	2179	7	10	NULL	0	NULL	GalCer	Process		binds					P1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25649_s_178	11940580	( If) as a function of P1 concentration exhibits a sharp transition between P1 concentration of 25 and 50 muM in both raft lipids and PBS environment, indicating that the GalCer* binding affinity to the P1 depends strongly on P1 concentration and, therefore, on P1 secondary structure (see Fig.  2).	bind
5374	2	2179	7	10	NULL	0	NULL	statement 1	Process		is dependent on 		strongly			P1	GP	concentration of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25649_s_178	11940580	( If) as a function of P1 concentration exhibits a sharp transition between P1 concentration of 25 and 50 muM in both raft lipids and PBS environment, indicating that the GalCer* binding affinity to the P1 depends strongly on P1 concentration and, therefore, on P1 secondary structure (see Fig.  2).	bind
5377	3	2179	7	10	NULL	0	NULL	statement 1	Process		is dependent on					P1	GP	secondary structure of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25649_s_178	11940580	( If) as a function of P1 concentration exhibits a sharp transition between P1 concentration of 25 and 50 muM in both raft lipids and PBS environment, indicating that the GalCer* binding affinity to the P1 depends strongly on P1 concentration and, therefore, on P1 secondary structure (see Fig.  2).	bind
3472	1	2180	6	10	NULL	0	NULL	TVA-EGF	GP		bind					M5 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_12_7063_s_137	9618539	( ii) A recombinant human EGF protein specifically blocked TVA-EGF binding to M5 cells and TVA-EGF mediated viral entry.	bind
3473	2	2180	6	10	NULL	0	NULL	EGF protein	GP	recombinant;;human	blocks		specifically			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_12_7063_s_137	9618539	( ii) A recombinant human EGF protein specifically blocked TVA-EGF binding to M5 cells and TVA-EGF mediated viral entry.	bind
3474	3	2180	6	10	NULL	0	NULL	TVA-EGF	GP		mediates					viral entry	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_12_7063_s_137	9618539	( ii) A recombinant human EGF protein specifically blocked TVA-EGF binding to M5 cells and TVA-EGF mediated viral entry.	bind
3475	4	2180	6	10	NULL	0	NULL	EGF protein	GP	recombinant;;human	blocks		specifically			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_12_7063_s_137	9618539	( ii) A recombinant human EGF protein specifically blocked TVA-EGF binding to M5 cells and TVA-EGF mediated viral entry.	bind
5378	1	2180	7	10	NULL	0	NULL	TVA-EGF	GP		binds					M5 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_12_7063_s_137	9618539	( ii) A recombinant human EGF protein specifically blocked TVA-EGF binding to M5 cells and TVA-EGF mediated viral entry.	bind
5379	2	2180	7	10	NULL	0	NULL	EGF protein 	GP	human;;recombinant	blocks		specifically			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_12_7063_s_137	9618539	( ii) A recombinant human EGF protein specifically blocked TVA-EGF binding to M5 cells and TVA-EGF mediated viral entry.	bind
5380	3	2180	7	10	NULL	0	NULL	TVA-EGF	GP		mediates					viral entry	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_12_7063_s_137	9618539	( ii) A recombinant human EGF protein specifically blocked TVA-EGF binding to M5 cells and TVA-EGF mediated viral entry.	bind
5381	4	2180	7	10	NULL	0	NULL	EGF protelin 	GP	human;;recombinant	blocks		specifically			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_12_7063_s_137	9618539	( ii) A recombinant human EGF protein specifically blocked TVA-EGF binding to M5 cells and TVA-EGF mediated viral entry.	bind
3476	1	2181	6	10	NULL	0	NULL	gp33	GP		bind					gp55 holoenzyme	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_50_17365_s_137	15574501	( ii) Binding of gp33 to gp55 holoenzyme was comparable with binding to core at low gp33 concentrations but reached saturation at higher gp33 concentrations ( Fig. 3 B).	bind
5382	1	2181	7	10	NULL	0	NULL	gp33 	GP		binds					gp55 holoenzyme	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_50_17365_s_137	15574501	( ii) Binding of gp33 to gp55 holoenzyme was comparable with binding to core at low gp33 concentrations but reached saturation at higher gp33 concentrations ( Fig. 3 B).	bind
3477	1	2182	6	10	NULL	0	NULL	eIF4F	GP		recognizes			eIF4E subunit		mRNA 	NucleicAcid			m7G cap at 5''-terminus	NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_13_7029_s_16	11416183	( ii) Binding of the 43S complex to mRNA, which in most instances occurs by a mechanism that involves initial recognition of the m7G cap at the mRNA 5''-terminus by the eIF4E (cap-binding) subunit of eIF4F.	bind
3478	2	2182	6	10	NULL	0	NULL	43S complex	GP		bind					mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_13_7029_s_16	11416183	( ii) Binding of the 43S complex to mRNA, which in most instances occurs by a mechanism that involves initial recognition of the m7G cap at the mRNA 5''-terminus by the eIF4E (cap-binding) subunit of eIF4F.	bind
3479	3	2182	6	10	NULL	0	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_13_7029_s_16	11416183	( ii) Binding of the 43S complex to mRNA, which in most instances occurs by a mechanism that involves initial recognition of the m7G cap at the mRNA 5''-terminus by the eIF4E (cap-binding) subunit of eIF4F.	bind
46035	4	2182	6	10	NULL	0	NULL	eIF4F	GP		is a type of			eIF4E subunit		cap-binding subunit	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_13_7029_s_16	11416183	( ii) Binding of the 43S complex to mRNA, which in most instances occurs by a mechanism that involves initial recognition of the m7G cap at the mRNA 5''-terminus by the eIF4E (cap-binding) subunit of eIF4F.	bind
5384	1	2182	7	10	NULL	0	NULL	43S complex	GP		binds					mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_13_7029_s_16	11416183	( ii) Binding of the 43S complex to mRNA, which in most instances occurs by a mechanism that involves initial recognition of the m7G cap at the mRNA 5''-terminus by the eIF4E (cap-binding) subunit of eIF4F.	bind
5385	2	2182	7	10	NULL	0	NULL	eIF4F	GP		recognizes			eIF4E subunit		mRNA	NucleicAcid			m7G cap at 5'' terminus	NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_13_7029_s_16	11416183	( ii) Binding of the 43S complex to mRNA, which in most instances occurs by a mechanism that involves initial recognition of the m7G cap at the mRNA 5''-terminus by the eIF4E (cap-binding) subunit of eIF4F.	bind
5386	3	2182	7	10	NULL	0	NULL	statement 1	Process		occurs by					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_13_7029_s_16	11416183	( ii) Binding of the 43S complex to mRNA, which in most instances occurs by a mechanism that involves initial recognition of the m7G cap at the mRNA 5''-terminus by the eIF4E (cap-binding) subunit of eIF4F.	bind
5387	4	2182	7	10	NULL	0	NULL	eIF4F	GP		is a type of			eIF4E subunit		cap-binding subunit	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_13_7029_s_16	11416183	( ii) Binding of the 43S complex to mRNA, which in most instances occurs by a mechanism that involves initial recognition of the m7G cap at the mRNA 5''-terminus by the eIF4E (cap-binding) subunit of eIF4F.	bind
3480	1	2183	6	10	NULL	0	NULL	AC	Chemical		bind					NPC1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_34_12473_s_163	15314240	( ii) Does the binding of [3]AC to NPC1 require the presence of NPC2?	bind
4398	2	2183	6	10	NULL	0	NULL	statement 1	Process		requires		possibly			NPC2	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_34_12473_s_163	15314240	( ii) Does the binding of [3]AC to NPC1 require the presence of NPC2?	bind
5388	1	2183	7	10	NULL	0	NULL	AC	Chemical		binds					NPC1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_34_12473_s_163	15314240	( ii) Does the binding of [3]AC to NPC1 require the presence of NPC2?	bind
46036	2	2183	7	10	NULL	0	NULL	statement 1	Process		requires		possibly			NPC2	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_34_12473_s_163	15314240	( ii) Does the binding of [3]AC to NPC1 require the presence of NPC2?	bind
3640	1	2185	6	10	NULL	0	NULL	Sp1	GP		does not bind					MYCN	GP			promoter	NULL	SH-EP cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_5110_s_265	14645238	( ii) Even prolonged treatment of 1A3 cells with 5-aC before induction with 4-OHT did not result in binding of E2F-1-ER or activation of endogenous  MYCN.( iii) In SH-EP cells, there was also no binding of Sp1 and Sp3 to the  MYCN promoter, although binding of Sp1 is not affected by methylation of DNA ( ).	bind
3641	2	2185	6	10	NULL	0	NULL	Sp3	GP		does not bind					MYCN	GP			promoter	NULL	SH-EP cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_5110_s_265	14645238	( ii) Even prolonged treatment of 1A3 cells with 5-aC before induction with 4-OHT did not result in binding of E2F-1-ER or activation of endogenous  MYCN.( iii) In SH-EP cells, there was also no binding of Sp1 and Sp3 to the  MYCN promoter, although binding of Sp1 is not affected by methylation of DNA ( ).	bind
3642	3	2185	6	10	NULL	0	NULL	DNA	NucleicAcid	methylation	does not affect					statement 1	Process				NULL	SH-EP cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_5110_s_265	14645238	( ii) Even prolonged treatment of 1A3 cells with 5-aC before induction with 4-OHT did not result in binding of E2F-1-ER or activation of endogenous  MYCN.( iii) In SH-EP cells, there was also no binding of Sp1 and Sp3 to the  MYCN promoter, although binding of Sp1 is not affected by methylation of DNA ( ).	bind
5399	1	2185	7	10	NULL	0	NULL	Sp1	GP		does not bind					MYCN	GP			promoter	NULL	in SH-EP cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_5110_s_265	14645238	( ii) Even prolonged treatment of 1A3 cells with 5-aC before induction with 4-OHT did not result in binding of E2F-1-ER or activation of endogenous  MYCN.( iii) In SH-EP cells, there was also no binding of Sp1 and Sp3 to the  MYCN promoter, although binding of Sp1 is not affected by methylation of DNA ( ).	bind
5400	2	2185	7	10	NULL	0	NULL	Sp3	GP		does not bind					MYCN	GP			promoter	NULL	in SH-EP cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_5110_s_265	14645238	( ii) Even prolonged treatment of 1A3 cells with 5-aC before induction with 4-OHT did not result in binding of E2F-1-ER or activation of endogenous  MYCN.( iii) In SH-EP cells, there was also no binding of Sp1 and Sp3 to the  MYCN promoter, although binding of Sp1 is not affected by methylation of DNA ( ).	bind
5401	3	2185	7	10	NULL	0	NULL	statement 1	Process		is not affected by					DNA	NucleicAcid	methylation of			NULL	in SH-EP cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_5110_s_265	14645238	( ii) Even prolonged treatment of 1A3 cells with 5-aC before induction with 4-OHT did not result in binding of E2F-1-ER or activation of endogenous  MYCN.( iii) In SH-EP cells, there was also no binding of Sp1 and Sp3 to the  MYCN promoter, although binding of Sp1 is not affected by methylation of DNA ( ).	bind
3570	1	2186	6	10	NULL	0	NULL	GroES	GP		bind					GroEL-polypeptide complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_21_12163_s_22	9770457	( ii) GroES binds to the GroEL-polypeptide complex, forming a  cis ternary complex in which the polypeptide is encapsulated within the GroEL-GroES structure ( 8-10).	bind
3571	2	2186	6	10	NULL	0	NULL	statement 1	Process		forms a					cis ternary complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_21_12163_s_22	9770457	( ii) GroES binds to the GroEL-polypeptide complex, forming a  cis ternary complex in which the polypeptide is encapsulated within the GroEL-GroES structure ( 8-10).	bind
51555	3	2186	6	10	NULL	0	NULL	polypeptide	GP		is  encapsulated within					GroEL-GroES	GP	structure of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_21_12163_s_22	9770457	( ii) GroES binds to the GroEL-polypeptide complex, forming a  cis ternary complex in which the polypeptide is encapsulated within the GroEL-GroES structure ( 8-10).	bind
51556	5	2186	6	10	NULL	0	NULL	statement 4	Process		is present in					cis ternary complex \t	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_21_12163_s_22	9770457	( ii) GroES binds to the GroEL-polypeptide complex, forming a  cis ternary complex in which the polypeptide is encapsulated within the GroEL-GroES structure ( 8-10).	bind
5402	1	2186	7	10	NULL	0	NULL	GroES	GP		binds to					GroEL-polypeptide complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_21_12163_s_22	9770457	( ii) GroES binds to the GroEL-polypeptide complex, forming a  cis ternary complex in which the polypeptide is encapsulated within the GroEL-GroES structure ( 8-10).	bind
5403	2	2186	7	10	NULL	0	NULL	statement 1	Process		forms					cis ternary complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_21_12163_s_22	9770457	( ii) GroES binds to the GroEL-polypeptide complex, forming a  cis ternary complex in which the polypeptide is encapsulated within the GroEL-GroES structure ( 8-10).	bind
5404	3	2186	7	10	NULL	0	NULL	polypeptide	GP		is  encapsulated within					GroEL-GroES	GP	structure of 			NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_21_12163_s_22	9770457	( ii) GroES binds to the GroEL-polypeptide complex, forming a  cis ternary complex in which the polypeptide is encapsulated within the GroEL-GroES structure ( 8-10).	bind
46037	4	2186	7	10	NULL	0	NULL	statement 4	Process		is present in					cis ternary complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_21_12163_s_22	9770457	( ii) GroES binds to the GroEL-polypeptide complex, forming a  cis ternary complex in which the polypeptide is encapsulated within the GroEL-GroES structure ( 8-10).	bind
3576	1	2187	6	10	NULL	0	NULL	ICP0	GP		bind			RING finger domain		cdc34	GP				NULL	in vitro substrate-independent ubiquitination system	NULL	NULL	NULL	NULL	gw60_pnas_98_15_8815_s_6	11447293	( ii) In an  in vitro substrate-independent ubiquitination system, the RING finger domain encoded by exon 2 of ICP0 binds cdc34, whereas the carboxyl-terminal domain of ICP0 functions as an E3 ligase independent of the RING finger domain.	bind
3577	2	2187	6	10	NULL	0	NULL	ICP0	GP		functions as			carboxyl-terminal domain		E3 ligase	GP				NULL	in vitro substrate-independent ubiquitination system	NULL	NULL	NULL	NULL	gw60_pnas_98_15_8815_s_6	11447293	( ii) In an  in vitro substrate-independent ubiquitination system, the RING finger domain encoded by exon 2 of ICP0 binds cdc34, whereas the carboxyl-terminal domain of ICP0 functions as an E3 ligase independent of the RING finger domain.	bind
3578	3	2187	6	10	NULL	0	NULL	statement 2	Process		independent of					ICP0	GP		RING finger domain		NULL	in vitro substrate-independent ubiquitination system	NULL	NULL	NULL	NULL	gw60_pnas_98_15_8815_s_6	11447293	( ii) In an  in vitro substrate-independent ubiquitination system, the RING finger domain encoded by exon 2 of ICP0 binds cdc34, whereas the carboxyl-terminal domain of ICP0 functions as an E3 ligase independent of the RING finger domain.	bind
3579	4	2187	6	10	NULL	0	NULL	ICP0	GP		encodes				exon 2	ICP0	GP		RING finger domain		NULL	in vitro substrate-independent ubiquitination system	NULL	NULL	NULL	NULL	gw60_pnas_98_15_8815_s_6	11447293	( ii) In an  in vitro substrate-independent ubiquitination system, the RING finger domain encoded by exon 2 of ICP0 binds cdc34, whereas the carboxyl-terminal domain of ICP0 functions as an E3 ligase independent of the RING finger domain.	bind
5405	1	2187	7	10	NULL	0	NULL	ICP0	GP		binds			RING finger domain		cdc34	GP				NULL	in vitro substrate-independent ubiquitination system	NULL	NULL	NULL	NULL	gw60_pnas_98_15_8815_s_6	11447293	( ii) In an  in vitro substrate-independent ubiquitination system, the RING finger domain encoded by exon 2 of ICP0 binds cdc34, whereas the carboxyl-terminal domain of ICP0 functions as an E3 ligase independent of the RING finger domain.	bind
5406	2	2187	7	10	NULL	0	NULL	ICP0	GP		functions as 			carboxyl-terminal domain 		E3 ligase	GP				NULL	in vitro substrate-independent ubiquitination system	NULL	NULL	NULL	NULL	gw60_pnas_98_15_8815_s_6	11447293	( ii) In an  in vitro substrate-independent ubiquitination system, the RING finger domain encoded by exon 2 of ICP0 binds cdc34, whereas the carboxyl-terminal domain of ICP0 functions as an E3 ligase independent of the RING finger domain.	bind
5407	3	2187	7	10	NULL	0	NULL	statement 2	Process		is independent of					ICP0	GP		RING finger domain		NULL	in vitro substrate-independent ubiquitination system	NULL	NULL	NULL	NULL	gw60_pnas_98_15_8815_s_6	11447293	( ii) In an  in vitro substrate-independent ubiquitination system, the RING finger domain encoded by exon 2 of ICP0 binds cdc34, whereas the carboxyl-terminal domain of ICP0 functions as an E3 ligase independent of the RING finger domain.	bind
5408	4	2187	7	10	NULL	0	NULL	ICP0	GP		is encoded by			RING finger domain		ICP0	GP			exon 2	NULL	in vitro substrate-independent ubiquitination system	NULL	NULL	NULL	NULL	gw60_pnas_98_15_8815_s_6	11447293	( ii) In an  in vitro substrate-independent ubiquitination system, the RING finger domain encoded by exon 2 of ICP0 binds cdc34, whereas the carboxyl-terminal domain of ICP0 functions as an E3 ligase independent of the RING finger domain.	bind
3580	1	2188	6	10	NULL	0	NULL	CCR5	GP		bind					MIP-1alpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_10_5740_s_32	9576954	( ii) It was reported that a complex of gp120 and soluble CD4 could inhibit binding between CCR5 and MIP-1alpha or MIP-1beta.	bind
3581	2	2188	6	10	NULL	0	NULL	CCR5	GP		bind					MIP-1beta	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_10_5740_s_32	9576954	( ii) It was reported that a complex of gp120 and soluble CD4 could inhibit binding between CCR5 and MIP-1alpha or MIP-1beta.	bind
3583	3	2188	6	10	NULL	0	NULL	gp120	GP		forms complex with					CD4	GP	soluble			NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_10_5740_s_32	9576954	( ii) It was reported that a complex of gp120 and soluble CD4 could inhibit binding between CCR5 and MIP-1alpha or MIP-1beta.	bind
3584	4	2188	6	10	NULL	0	NULL	statement 3	Process		inhibit		probably			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_10_5740_s_32	9576954	( ii) It was reported that a complex of gp120 and soluble CD4 could inhibit binding between CCR5 and MIP-1alpha or MIP-1beta.	bind
3585	5	2188	6	10	NULL	0	NULL	statement 3	Process		inhibit		probably			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_10_5740_s_32	9576954	( ii) It was reported that a complex of gp120 and soluble CD4 could inhibit binding between CCR5 and MIP-1alpha or MIP-1beta.	bind
5411	1	2188	7	10	NULL	0	NULL	CCR5	GP		binds					MIP-1alpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_10_5740_s_32	9576954	( ii) It was reported that a complex of gp120 and soluble CD4 could inhibit binding between CCR5 and MIP-1alpha or MIP-1beta.	bind
5412	2	2188	7	10	NULL	0	NULL	CCR5	GP		binds					MIP-1beta	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_10_5740_s_32	9576954	( ii) It was reported that a complex of gp120 and soluble CD4 could inhibit binding between CCR5 and MIP-1alpha or MIP-1beta.	bind
5413	3	2188	7	10	NULL	0	NULL	 gp120	GP		forms complex with					CD4	GP	soluble			NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_10_5740_s_32	9576954	( ii) It was reported that a complex of gp120 and soluble CD4 could inhibit binding between CCR5 and MIP-1alpha or MIP-1beta.	bind
5414	4	2188	7	10	NULL	0	NULL	statement 3	Process		inhibit		may			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_10_5740_s_32	9576954	( ii) It was reported that a complex of gp120 and soluble CD4 could inhibit binding between CCR5 and MIP-1alpha or MIP-1beta.	bind
5415	5	2188	7	10	NULL	0	NULL	statement 3	Process		inhibit		may			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_10_5740_s_32	9576954	( ii) It was reported that a complex of gp120 and soluble CD4 could inhibit binding between CCR5 and MIP-1alpha or MIP-1beta.	bind
3586	1	2189	6	10	NULL	0	NULL	nucleosomes	Chromosome		bind		may	H3.1		nucleosomes	Chromosome		H3.1		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_17_6428_s_114	16571659	( ii) Nucleosomes that contain H3.1 might bind to other H3.1-containing nucleosomes through internucleosomal disulfide bonds between cysteines 96.	bind
3587	2	2189	6	10	NULL	0	NULL	statement 1	Process		occurs through					disulfide bonds		internucleosomal	cysteines 96		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_17_6428_s_114	16571659	( ii) Nucleosomes that contain H3.1 might bind to other H3.1-containing nucleosomes through internucleosomal disulfide bonds between cysteines 96.	bind
5417	1	2189	7	10	NULL	0	NULL	nucleosomes	Chromosome		bind		may	H3.1		nucleosomes	Chromosome		H3.1		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_17_6428_s_114	16571659	( ii) Nucleosomes that contain H3.1 might bind to other H3.1-containing nucleosomes through internucleosomal disulfide bonds between cysteines 96.	bind
46342	2	2189	7	10	NULL	0	NULL	statement 1	Process		occurs through					disulfide bonds		internucleosomal	cysteines 96		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_17_6428_s_114	16571659	( ii) Nucleosomes that contain H3.1 might bind to other H3.1-containing nucleosomes through internucleosomal disulfide bonds between cysteines 96.	bind
3588	1	2190	6	10	NULL	0	NULL	MHC peptide complex	GP		are present on					B cells	Cell				NULL	B cells and APCs	NULL	NULL	NULL	NULL	gw70_pnas_102_18_6245_s_74	15843460	( ii) T cells recognize and bind to the MHC peptide complex on B cells and APCs. ( iii) B cells are stimulated, either directly by T cell binding or indirectly through  the bystander effect.	bind
3589	2	2190	6	10	NULL	0	NULL	MHC peptide complex	GP		is present at					APC	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_18_6245_s_74	15843460	( ii) T cells recognize and bind to the MHC peptide complex on B cells and APCs. ( iii) B cells are stimulated, either directly by T cell binding or indirectly through  the bystander effect.	bind
3590	3	2190	6	10	NULL	0	NULL	T cells	Cell	binding of	stimulate		directly			B cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_18_6245_s_74	15843460	( ii) T cells recognize and bind to the MHC peptide complex on B cells and APCs. ( iii) B cells are stimulated, either directly by T cell binding or indirectly through  the bystander effect.	bind
3591	4	2190	6	10	NULL	0	NULL	bystander effect	Process		stimulate		indirectly			B cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_18_6245_s_74	15843460	( ii) T cells recognize and bind to the MHC peptide complex on B cells and APCs. ( iii) B cells are stimulated, either directly by T cell binding or indirectly through  the bystander effect.	bind
46301	5	2190	6	10	NULL	0	NULL	T cells	Cell		recognize					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_18_6245_s_74	15843460	( ii) T cells recognize and bind to the MHC peptide complex on B cells and APCs. ( iii) B cells are stimulated, either directly by T cell binding or indirectly through  the bystander effect.	bind
46302	6	2190	6	10	NULL	0	NULL	T cell	Cell		recognize					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_18_6245_s_74	15843460	( ii) T cells recognize and bind to the MHC peptide complex on B cells and APCs. ( iii) B cells are stimulated, either directly by T cell binding or indirectly through  the bystander effect.	bind
46303	7	2190	6	10	NULL	0	NULL	T cells	Cell		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_18_6245_s_74	15843460	( ii) T cells recognize and bind to the MHC peptide complex on B cells and APCs. ( iii) B cells are stimulated, either directly by T cell binding or indirectly through  the bystander effect.	bind
46304	8	2190	6	10	NULL	0	NULL	T cells	Cell		bind					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_18_6245_s_74	15843460	( ii) T cells recognize and bind to the MHC peptide complex on B cells and APCs. ( iii) B cells are stimulated, either directly by T cell binding or indirectly through  the bystander effect.	bind
5419	1	2190	7	10	NULL	0	NULL	MHC peptide complex	GP		is present at					B cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_18_6245_s_74	15843460	( ii) T cells recognize and bind to the MHC peptide complex on B cells and APCs. ( iii) B cells are stimulated, either directly by T cell binding or indirectly through  the bystander effect.	bind
5420	2	2190	7	10	NULL	0	NULL	MHC peptide complex	GP		is present at					APCs	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_18_6245_s_74	15843460	( ii) T cells recognize and bind to the MHC peptide complex on B cells and APCs. ( iii) B cells are stimulated, either directly by T cell binding or indirectly through  the bystander effect.	bind
5421	3	2190	7	10	NULL	0	NULL	T cells	Cell		recognize					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_18_6245_s_74	15843460	( ii) T cells recognize and bind to the MHC peptide complex on B cells and APCs. ( iii) B cells are stimulated, either directly by T cell binding or indirectly through  the bystander effect.	bind
5422	4	2190	7	10	NULL	0	NULL	T cells 	Cell		recognize					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_18_6245_s_74	15843460	( ii) T cells recognize and bind to the MHC peptide complex on B cells and APCs. ( iii) B cells are stimulated, either directly by T cell binding or indirectly through  the bystander effect.	bind
46343	5	2190	7	10	NULL	0	NULL	T cells	Cell		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_18_6245_s_74	15843460	( ii) T cells recognize and bind to the MHC peptide complex on B cells and APCs. ( iii) B cells are stimulated, either directly by T cell binding or indirectly through  the bystander effect.	bind
46344	6	2190	7	10	NULL	0	NULL	T cells	Cell		bind					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_18_6245_s_74	15843460	( ii) T cells recognize and bind to the MHC peptide complex on B cells and APCs. ( iii) B cells are stimulated, either directly by T cell binding or indirectly through  the bystander effect.	bind
46345	7	2190	7	10	NULL	0	NULL	T cells	Cell	binding of	stimulate		directly			B cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_18_6245_s_74	15843460	( ii) T cells recognize and bind to the MHC peptide complex on B cells and APCs. ( iii) B cells are stimulated, either directly by T cell binding or indirectly through  the bystander effect.	bind
46346	8	2190	7	10	NULL	0	NULL	bystander effect	Process		stimulate		indirectly			B cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_18_6245_s_74	15843460	( ii) T cells recognize and bind to the MHC peptide complex on B cells and APCs. ( iii) B cells are stimulated, either directly by T cell binding or indirectly through  the bystander effect.	bind
3592	1	2192	6	10	NULL	0	NULL	PP1	GP	purified	does not bind			C subunit		GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_20_10624_s_104	9380685	( ii) The purified C subunit of PP1 did not show binding to either GST or GST-alpha4 (Fig.  1 c).	bind
3593	2	2192	6	10	NULL	0	NULL	PP1	GP	purified	does not bind			C subunit		GST-alpha4	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_20_10624_s_104	9380685	( ii) The purified C subunit of PP1 did not show binding to either GST or GST-alpha4 (Fig.  1 c).	bind
5423	1	2192	7	10	NULL	0	NULL	PP1	GP	purified	does not bind			C subunit 		GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_20_10624_s_104	9380685	( ii) The purified C subunit of PP1 did not show binding to either GST or GST-alpha4 (Fig.  1 c).	bind
5424	2	2192	7	10	NULL	0	NULL	PP1	GP	purified	does not bind			C subunit 		GST-alpha4	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_20_10624_s_104	9380685	( ii) The purified C subunit of PP1 did not show binding to either GST or GST-alpha4 (Fig.  1 c).	bind
3594	1	2193	6	10	NULL	0	NULL	X5	GP		bind					gp120	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_10_6913_s_176	11997472	( ii) X5 binding to gp120 was enhanced by the A32 mAb, which binds a CD4-inducible epitope; in turn X5 binding enhanced the exposure of the A32 epitope (data not shown).	bind
3595	2	2193	6	10	NULL	0	NULL	statement 1	Process		enhanced by					A32 mAb	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_10_6913_s_176	11997472	( ii) X5 binding to gp120 was enhanced by the A32 mAb, which binds a CD4-inducible epitope; in turn X5 binding enhanced the exposure of the A32 epitope (data not shown).	bind
3596	3	2193	6	10	NULL	0	NULL	A32 mAb	GP		bind					CD4-inducible epitope					NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_10_6913_s_176	11997472	( ii) X5 binding to gp120 was enhanced by the A32 mAb, which binds a CD4-inducible epitope; in turn X5 binding enhanced the exposure of the A32 epitope (data not shown).	bind
3597	4	2193	6	10	NULL	0	NULL	statement 1	Process		enhance					A32 epitope		exposure of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_10_6913_s_176	11997472	( ii) X5 binding to gp120 was enhanced by the A32 mAb, which binds a CD4-inducible epitope; in turn X5 binding enhanced the exposure of the A32 epitope (data not shown).	bind
5425	1	2193	7	10	NULL	0	NULL	X5	GP		binds to					gp120	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_10_6913_s_176	11997472	( ii) X5 binding to gp120 was enhanced by the A32 mAb, which binds a CD4-inducible epitope; in turn X5 binding enhanced the exposure of the A32 epitope (data not shown).	bind
5426	2	2193	7	10	NULL	0	NULL	statement 1	Process		is enhanced by					A32 mAb	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_10_6913_s_176	11997472	( ii) X5 binding to gp120 was enhanced by the A32 mAb, which binds a CD4-inducible epitope; in turn X5 binding enhanced the exposure of the A32 epitope (data not shown).	bind
5427	3	2193	7	10	NULL	0	NULL	A32 mAb	GP		binds					CD4-inducible epitope					NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_10_6913_s_176	11997472	( ii) X5 binding to gp120 was enhanced by the A32 mAb, which binds a CD4-inducible epitope; in turn X5 binding enhanced the exposure of the A32 epitope (data not shown).	bind
5428	4	2193	7	10	NULL	0	NULL	statement 1	Process		enhanced 					A32 epitope		exposure of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_10_6913_s_176	11997472	( ii) X5 binding to gp120 was enhanced by the A32 mAb, which binds a CD4-inducible epitope; in turn X5 binding enhanced the exposure of the A32 epitope (data not shown).	bind
3598	1	2195	6	10	NULL	0	NULL	NPC2	GP		bind		may			membranes	CellComponent	cholesterol rich			NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_5_2518_s_318	12591949	( iii) NPC2 could bind to cholesterol-rich membranes and, through protein-protein interactions, could influence the localization of other proteins, such as NPC1, that mobilize lipids.	bind
3599	2	2195	6	10	NULL	0	NULL	statement 1	Process		influence 		may			NPC1	GP	localization of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_5_2518_s_318	12591949	( iii) NPC2 could bind to cholesterol-rich membranes and, through protein-protein interactions, could influence the localization of other proteins, such as NPC1, that mobilize lipids.	bind
3600	3	2195	6	10	NULL	0	NULL	NPC1	GP		mobilize					lipids	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_5_2518_s_318	12591949	( iii) NPC2 could bind to cholesterol-rich membranes and, through protein-protein interactions, could influence the localization of other proteins, such as NPC1, that mobilize lipids.	bind
5429	1	2195	7	10	NULL	0	NULL	NPC2	GP		bind to		could			membranes	CellComponent	cholesterol-rich 			NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_5_2518_s_318	12591949	( iii) NPC2 could bind to cholesterol-rich membranes and, through protein-protein interactions, could influence the localization of other proteins, such as NPC1, that mobilize lipids.	bind
5431	2	2195	7	10	NULL	0	NULL	statement 1	Process		influence		could			NPC1	GP	localization of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_5_2518_s_318	12591949	( iii) NPC2 could bind to cholesterol-rich membranes and, through protein-protein interactions, could influence the localization of other proteins, such as NPC1, that mobilize lipids.	bind
5434	3	2195	7	10	NULL	0	NULL	NPC1	GP		mobilize					lipids	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_5_2518_s_318	12591949	( iii) NPC2 could bind to cholesterol-rich membranes and, through protein-protein interactions, could influence the localization of other proteins, such as NPC1, that mobilize lipids.	bind
3601	1	2196	6	10	NULL	0	NULL	GTP[gamma35] 	Chemical		bind					platelet membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_16_8750_s_167	9238049	( iii) The binding of GTP[gamma35] to patient platelet membranes in response to thrombin stimulation was markedly diminished.	bind
3602	2	2196	6	10	NULL	0	NULL	statement 1	Process		in response to					thrombin	GP	stimulation			NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_16_8750_s_167	9238049	( iii) The binding of GTP[gamma35] to patient platelet membranes in response to thrombin stimulation was markedly diminished.	bind
5436	1	2196	7	10	NULL	0	NULL	GTP[gamma35]	Chemical		binds to					platelet membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_16_8750_s_167	9238049	( iii) The binding of GTP[gamma35] to patient platelet membranes in response to thrombin stimulation was markedly diminished.	bind
5437	2	2196	7	10	NULL	0	NULL	Thrombin	GP	stimulation of	leads to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_16_8750_s_167	9238049	( iii) The binding of GTP[gamma35] to patient platelet membranes in response to thrombin stimulation was markedly diminished.	bind
3604	2	2197	6	10	NULL	0	NULL	anti-8-nitroguanosine antibody	GP		bind					8-nitroguanosine-BSA conjugate	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_2_685_s_81	12522148	( Inset) Binding of anti-8-nitroguanosine antibody to BSA or 8-nitroguanosine-BSA conjugate  fixed on microtiter plates.	bind
46294	1	2197	6	10	NULL	0	NULL	anti-8-nitroguanosine antibody	GP		bind					BSA	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_2_685_s_81	12522148	( Inset) Binding of anti-8-nitroguanosine antibody to BSA or 8-nitroguanosine-BSA conjugate  fixed on microtiter plates.	bind
5440	1	2197	7	10	NULL	0	NULL	anti-8-nitroguanosine antibody	GP		bind					BSA	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_2_685_s_81	12522148	( Inset) Binding of anti-8-nitroguanosine antibody to BSA or 8-nitroguanosine-BSA conjugate  fixed on microtiter plates.	bind
46295	2	2197	7	10	NULL	0	NULL	 anti-8-nitroguanosine antibody 	GP		bind					 8-nitroguanosine-BSA	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_2_685_s_81	12522148	( Inset) Binding of anti-8-nitroguanosine antibody to BSA or 8-nitroguanosine-BSA conjugate  fixed on microtiter plates.	bind
3643	1	2199	6	10	NULL	0	NULL	bicuculline	Chemical		blocks					BTX	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_41	16549768	( Inset) Double-reciprocal plot shows that  Kd  50 nM. ( b) BTX binding to this cell line was insensitive to preincubation with blockers of  nAChRs containing alpha1 or alpha7 subunits [methyllycaconitine (MLA), nicotine (Nic), and hexamethonium (Hexa)] or  the GABAAR modulator pentobarbital (PB) but was blocked by the GABAAR antagonist bicuculline (Bic).	bind
3644	2	2199	6	10	NULL	0	NULL	Bic	Chemical		is					bicuculline	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_41	16549768	( Inset) Double-reciprocal plot shows that  Kd  50 nM. ( b) BTX binding to this cell line was insensitive to preincubation with blockers of  nAChRs containing alpha1 or alpha7 subunits [methyllycaconitine (MLA), nicotine (Nic), and hexamethonium (Hexa)] or  the GABAAR modulator pentobarbital (PB) but was blocked by the GABAAR antagonist bicuculline (Bic).	bind
46062	3	2199	6	10	NULL	0	NULL	bicuculline	Chemical		is an antagonist of					GABAAR	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_41	16549768	( Inset) Double-reciprocal plot shows that  Kd  50 nM. ( b) BTX binding to this cell line was insensitive to preincubation with blockers of  nAChRs containing alpha1 or alpha7 subunits [methyllycaconitine (MLA), nicotine (Nic), and hexamethonium (Hexa)] or  the GABAAR modulator pentobarbital (PB) but was blocked by the GABAAR antagonist bicuculline (Bic).	bind
46305	4	2199	6	10	NULL	0	NULL	MLA	Chemical		is					methyllycaconitine	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_41	16549768	( Inset) Double-reciprocal plot shows that  Kd  50 nM. ( b) BTX binding to this cell line was insensitive to preincubation with blockers of  nAChRs containing alpha1 or alpha7 subunits [methyllycaconitine (MLA), nicotine (Nic), and hexamethonium (Hexa)] or  the GABAAR modulator pentobarbital (PB) but was blocked by the GABAAR antagonist bicuculline (Bic).	bind
46306	5	2199	6	10	NULL	0	NULL	Nic	Chemical		is					nicotine	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_41	16549768	( Inset) Double-reciprocal plot shows that  Kd  50 nM. ( b) BTX binding to this cell line was insensitive to preincubation with blockers of  nAChRs containing alpha1 or alpha7 subunits [methyllycaconitine (MLA), nicotine (Nic), and hexamethonium (Hexa)] or  the GABAAR modulator pentobarbital (PB) but was blocked by the GABAAR antagonist bicuculline (Bic).	bind
46307	6	2199	6	10	NULL	0	NULL	Hexa	Chemical		is					hexamethonium	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_41	16549768	( Inset) Double-reciprocal plot shows that  Kd  50 nM. ( b) BTX binding to this cell line was insensitive to preincubation with blockers of  nAChRs containing alpha1 or alpha7 subunits [methyllycaconitine (MLA), nicotine (Nic), and hexamethonium (Hexa)] or  the GABAAR modulator pentobarbital (PB) but was blocked by the GABAAR antagonist bicuculline (Bic).	bind
46308	7	2199	6	10	NULL	0	NULL	PB	Chemical		is					pentobarbital	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_41	16549768	( Inset) Double-reciprocal plot shows that  Kd  50 nM. ( b) BTX binding to this cell line was insensitive to preincubation with blockers of  nAChRs containing alpha1 or alpha7 subunits [methyllycaconitine (MLA), nicotine (Nic), and hexamethonium (Hexa)] or  the GABAAR modulator pentobarbital (PB) but was blocked by the GABAAR antagonist bicuculline (Bic).	bind
46309	8	2199	6	10	NULL	0	NULL	pentobarbital	Chemical		is a type of					GABAAR modulator 	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_41	16549768	( Inset) Double-reciprocal plot shows that  Kd  50 nM. ( b) BTX binding to this cell line was insensitive to preincubation with blockers of  nAChRs containing alpha1 or alpha7 subunits [methyllycaconitine (MLA), nicotine (Nic), and hexamethonium (Hexa)] or  the GABAAR modulator pentobarbital (PB) but was blocked by the GABAAR antagonist bicuculline (Bic).	bind
51557	9	2199	6	10	NULL	0	NULL	MLA	Chemical		is a type of					nAChR blocker	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_41	16549768	( Inset) Double-reciprocal plot shows that  Kd  50 nM. ( b) BTX binding to this cell line was insensitive to preincubation with blockers of  nAChRs containing alpha1 or alpha7 subunits [methyllycaconitine (MLA), nicotine (Nic), and hexamethonium (Hexa)] or  the GABAAR modulator pentobarbital (PB) but was blocked by the GABAAR antagonist bicuculline (Bic).	bind
51558	10	2199	6	10	NULL	0	NULL	Nic	Chemical		is a type of					nAChR blocker	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_41	16549768	( Inset) Double-reciprocal plot shows that  Kd  50 nM. ( b) BTX binding to this cell line was insensitive to preincubation with blockers of  nAChRs containing alpha1 or alpha7 subunits [methyllycaconitine (MLA), nicotine (Nic), and hexamethonium (Hexa)] or  the GABAAR modulator pentobarbital (PB) but was blocked by the GABAAR antagonist bicuculline (Bic).	bind
51559	11	2199	6	10	NULL	0	NULL	Hexa	Chemical		is a type of					nAChR blocker	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_41	16549768	( Inset) Double-reciprocal plot shows that  Kd  50 nM. ( b) BTX binding to this cell line was insensitive to preincubation with blockers of  nAChRs containing alpha1 or alpha7 subunits [methyllycaconitine (MLA), nicotine (Nic), and hexamethonium (Hexa)] or  the GABAAR modulator pentobarbital (PB) but was blocked by the GABAAR antagonist bicuculline (Bic).	bind
6320	2	2199	7	10	NULL	0	NULL	MLA	Chemical		is					methyllycaconitine	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_41	16549768	( Inset) Double-reciprocal plot shows that  Kd  50 nM. ( b) BTX binding to this cell line was insensitive to preincubation with blockers of  nAChRs containing alpha1 or alpha7 subunits [methyllycaconitine (MLA), nicotine (Nic), and hexamethonium (Hexa)] or  the GABAAR modulator pentobarbital (PB) but was blocked by the GABAAR antagonist bicuculline (Bic).	bind
6321	3	2199	7	10	NULL	0	NULL	Nic	Chemical		is					nicotine	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_41	16549768	( Inset) Double-reciprocal plot shows that  Kd  50 nM. ( b) BTX binding to this cell line was insensitive to preincubation with blockers of  nAChRs containing alpha1 or alpha7 subunits [methyllycaconitine (MLA), nicotine (Nic), and hexamethonium (Hexa)] or  the GABAAR modulator pentobarbital (PB) but was blocked by the GABAAR antagonist bicuculline (Bic).	bind
6322	4	2199	7	10	NULL	0	NULL	hexa	Chemical		is					hexamethonium	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_41	16549768	( Inset) Double-reciprocal plot shows that  Kd  50 nM. ( b) BTX binding to this cell line was insensitive to preincubation with blockers of  nAChRs containing alpha1 or alpha7 subunits [methyllycaconitine (MLA), nicotine (Nic), and hexamethonium (Hexa)] or  the GABAAR modulator pentobarbital (PB) but was blocked by the GABAAR antagonist bicuculline (Bic).	bind
6323	5	2199	7	10	NULL	0	NULL	PB	Chemical		is					pentobarbital	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_41	16549768	( Inset) Double-reciprocal plot shows that  Kd  50 nM. ( b) BTX binding to this cell line was insensitive to preincubation with blockers of  nAChRs containing alpha1 or alpha7 subunits [methyllycaconitine (MLA), nicotine (Nic), and hexamethonium (Hexa)] or  the GABAAR modulator pentobarbital (PB) but was blocked by the GABAAR antagonist bicuculline (Bic).	bind
6324	6	2199	7	10	NULL	0	NULL	pentobarbital	Chemical		is a type of					GABAAR modulator	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_41	16549768	( Inset) Double-reciprocal plot shows that  Kd  50 nM. ( b) BTX binding to this cell line was insensitive to preincubation with blockers of  nAChRs containing alpha1 or alpha7 subunits [methyllycaconitine (MLA), nicotine (Nic), and hexamethonium (Hexa)] or  the GABAAR modulator pentobarbital (PB) but was blocked by the GABAAR antagonist bicuculline (Bic).	bind
6325	7	2199	7	10	NULL	0	NULL	Bic	Chemical		is					bicuculline	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_41	16549768	( Inset) Double-reciprocal plot shows that  Kd  50 nM. ( b) BTX binding to this cell line was insensitive to preincubation with blockers of  nAChRs containing alpha1 or alpha7 subunits [methyllycaconitine (MLA), nicotine (Nic), and hexamethonium (Hexa)] or  the GABAAR modulator pentobarbital (PB) but was blocked by the GABAAR antagonist bicuculline (Bic).	bind
6326	8	2199	7	10	NULL	0	NULL	bicuculline	Chemical		is antagonist of					GABAAR	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_41	16549768	( Inset) Double-reciprocal plot shows that  Kd  50 nM. ( b) BTX binding to this cell line was insensitive to preincubation with blockers of  nAChRs containing alpha1 or alpha7 subunits [methyllycaconitine (MLA), nicotine (Nic), and hexamethonium (Hexa)] or  the GABAAR modulator pentobarbital (PB) but was blocked by the GABAAR antagonist bicuculline (Bic).	bind
6327	9	2199	7	10	NULL	0	NULL	MLA	Chemical		is a type of					nAChR blocker	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_41	16549768	( Inset) Double-reciprocal plot shows that  Kd  50 nM. ( b) BTX binding to this cell line was insensitive to preincubation with blockers of  nAChRs containing alpha1 or alpha7 subunits [methyllycaconitine (MLA), nicotine (Nic), and hexamethonium (Hexa)] or  the GABAAR modulator pentobarbital (PB) but was blocked by the GABAAR antagonist bicuculline (Bic).	bind
6328	10	2199	7	10	NULL	0	NULL	Nic	Chemical		is a type of					nAChR blocker	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_41	16549768	( Inset) Double-reciprocal plot shows that  Kd  50 nM. ( b) BTX binding to this cell line was insensitive to preincubation with blockers of  nAChRs containing alpha1 or alpha7 subunits [methyllycaconitine (MLA), nicotine (Nic), and hexamethonium (Hexa)] or  the GABAAR modulator pentobarbital (PB) but was blocked by the GABAAR antagonist bicuculline (Bic).	bind
6329	11	2199	7	10	NULL	0	NULL	hexa	Chemical		is a type of					nAChR blocker	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_41	16549768	( Inset) Double-reciprocal plot shows that  Kd  50 nM. ( b) BTX binding to this cell line was insensitive to preincubation with blockers of  nAChRs containing alpha1 or alpha7 subunits [methyllycaconitine (MLA), nicotine (Nic), and hexamethonium (Hexa)] or  the GABAAR modulator pentobarbital (PB) but was blocked by the GABAAR antagonist bicuculline (Bic).	bind
46347	1	2199	7	10	NULL	0	NULL	Bic	Chemical		blocks					BTX	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_13_5149_s_41	16549768	( Inset) Double-reciprocal plot shows that  Kd  50 nM. ( b) BTX binding to this cell line was insensitive to preincubation with blockers of  nAChRs containing alpha1 or alpha7 subunits [methyllycaconitine (MLA), nicotine (Nic), and hexamethonium (Hexa)] or  the GABAAR modulator pentobarbital (PB) but was blocked by the GABAAR antagonist bicuculline (Bic).	bind
3605	1	2200	6	10	NULL	0	NULL	RecA	GP	wild type	bind					p/t DNA	NucleicAcid			15-nt oh	NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_17_11061_s_117	12177433	( Inset) The data depict wild-type RecA binding to p/t DNA with a 15-nt oh; RecA protein binding to p/t DNA with a 12-nt oh; RecA 1730 protein binding to p/t with a 15-nt oh; RecA1730 protein binding to p/t with a 12-nt oh.	bind
3606	2	2200	6	10	NULL	0	NULL	RecA protein	GP		bind					p/t DNA	NucleicAcid			12-nt oh	NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_17_11061_s_117	12177433	( Inset) The data depict wild-type RecA binding to p/t DNA with a 15-nt oh; RecA protein binding to p/t DNA with a 12-nt oh; RecA 1730 protein binding to p/t with a 15-nt oh; RecA1730 protein binding to p/t with a 12-nt oh.	bind
3607	3	2200	6	10	NULL	0	NULL	RecA 1730 protein	GP		bind					p/t DNA	NucleicAcid			15-nt oh	NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_17_11061_s_117	12177433	( Inset) The data depict wild-type RecA binding to p/t DNA with a 15-nt oh; RecA protein binding to p/t DNA with a 12-nt oh; RecA 1730 protein binding to p/t with a 15-nt oh; RecA1730 protein binding to p/t with a 12-nt oh.	bind
3608	4	2200	6	10	NULL	0	NULL	RecA 1730 protein	GP		bind					p/t DNA	NucleicAcid			12-nt oh	NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_17_11061_s_117	12177433	( Inset) The data depict wild-type RecA binding to p/t DNA with a 15-nt oh; RecA protein binding to p/t DNA with a 12-nt oh; RecA 1730 protein binding to p/t with a 15-nt oh; RecA1730 protein binding to p/t with a 12-nt oh.	bind
5464	1	2200	7	10	NULL	0	NULL	RecA	GP	Wild-type	binds to					p/t DNA	NucleicAcid			15-nt oh	NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_17_11061_s_117	12177433	( Inset) The data depict wild-type RecA binding to p/t DNA with a 15-nt oh; RecA protein binding to p/t DNA with a 12-nt oh; RecA 1730 protein binding to p/t with a 15-nt oh; RecA1730 protein binding to p/t with a 12-nt oh.	bind
5466	2	2200	7	10	NULL	0	NULL	RecA protein	GP		binds to					p/t DNA	NucleicAcid			12-nt oh	NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_17_11061_s_117	12177433	( Inset) The data depict wild-type RecA binding to p/t DNA with a 15-nt oh; RecA protein binding to p/t DNA with a 12-nt oh; RecA 1730 protein binding to p/t with a 15-nt oh; RecA1730 protein binding to p/t with a 12-nt oh.	bind
5468	3	2200	7	10	NULL	0	NULL	RecA 1730 protein	GP		binds to					p/t DNA	NucleicAcid			15-nt oh	NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_17_11061_s_117	12177433	( Inset) The data depict wild-type RecA binding to p/t DNA with a 15-nt oh; RecA protein binding to p/t DNA with a 12-nt oh; RecA 1730 protein binding to p/t with a 15-nt oh; RecA1730 protein binding to p/t with a 12-nt oh.	bind
5471	4	2200	7	10	NULL	0	NULL	RecA1730 protein	GP		binds to					p/t DNA	NucleicAcid			12-nt oh	NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_17_11061_s_117	12177433	( Inset) The data depict wild-type RecA binding to p/t DNA with a 15-nt oh; RecA protein binding to p/t DNA with a 12-nt oh; RecA 1730 protein binding to p/t with a 15-nt oh; RecA1730 protein binding to p/t with a 12-nt oh.	bind
3766	1	2202	5	10	NULL	0	NULL	IRp antibody	GP		bind					IR	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_21_11692_s_142	9326672	( iv) An antibody to IRp binds to IR (but not to a deletion mutant of IR or to IGF-1R), inhibits insulin-induced internalization of IR, enhances insulin-stimulated glucose uptake, and competes with IRp for binding.	bind
3767	2	2202	5	10	NULL	0	NULL	IRp antibody	GP		does not bind					IR	GP	deletion mutant			NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_21_11692_s_142	9326672	( iv) An antibody to IRp binds to IR (but not to a deletion mutant of IR or to IGF-1R), inhibits insulin-induced internalization of IR, enhances insulin-stimulated glucose uptake, and competes with IRp for binding.	bind
3768	3	2202	5	10	NULL	0	NULL	IRp antibody	GP		does not bind					IGF-1R	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_21_11692_s_142	9326672	( iv) An antibody to IRp binds to IR (but not to a deletion mutant of IR or to IGF-1R), inhibits insulin-induced internalization of IR, enhances insulin-stimulated glucose uptake, and competes with IRp for binding.	bind
3769	4	2202	5	10	NULL	0	NULL	insulin	GP		induce					IR	GP	internalization of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_21_11692_s_142	9326672	( iv) An antibody to IRp binds to IR (but not to a deletion mutant of IR or to IGF-1R), inhibits insulin-induced internalization of IR, enhances insulin-stimulated glucose uptake, and competes with IRp for binding.	bind
3770	5	2202	5	10	NULL	0	NULL	IRp antibody	GP		inhibit					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_21_11692_s_142	9326672	( iv) An antibody to IRp binds to IR (but not to a deletion mutant of IR or to IGF-1R), inhibits insulin-induced internalization of IR, enhances insulin-stimulated glucose uptake, and competes with IRp for binding.	bind
3771	6	2202	5	10	NULL	0	NULL	insulin	GP		stimulate					glucose uptake	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_21_11692_s_142	9326672	( iv) An antibody to IRp binds to IR (but not to a deletion mutant of IR or to IGF-1R), inhibits insulin-induced internalization of IR, enhances insulin-stimulated glucose uptake, and competes with IRp for binding.	bind
3772	7	2202	5	10	NULL	0	NULL	IRp antibody	GP		enhance					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_21_11692_s_142	9326672	( iv) An antibody to IRp binds to IR (but not to a deletion mutant of IR or to IGF-1R), inhibits insulin-induced internalization of IR, enhances insulin-stimulated glucose uptake, and competes with IRp for binding.	bind
3773	8	2202	5	10	NULL	0	NULL	IRp	GP		bind					IR	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_21_11692_s_142	9326672	( iv) An antibody to IRp binds to IR (but not to a deletion mutant of IR or to IGF-1R), inhibits insulin-induced internalization of IR, enhances insulin-stimulated glucose uptake, and competes with IRp for binding.	bind
3774	9	2202	5	10	NULL	0	NULL	statement 1	Process		compete with					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_21_11692_s_142	9326672	( iv) An antibody to IRp binds to IR (but not to a deletion mutant of IR or to IGF-1R), inhibits insulin-induced internalization of IR, enhances insulin-stimulated glucose uptake, and competes with IRp for binding.	bind
3609	1	2202	6	10	NULL	0	NULL	IRp antibody	GP		bind					IR	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_21_11692_s_142	9326672	( iv) An antibody to IRp binds to IR (but not to a deletion mutant of IR or to IGF-1R), inhibits insulin-induced internalization of IR, enhances insulin-stimulated glucose uptake, and competes with IRp for binding.	bind
3610	2	2202	6	10	NULL	0	NULL	IRp antibody	GP		does not bind					IR	GP	deletion mutant			NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_21_11692_s_142	9326672	( iv) An antibody to IRp binds to IR (but not to a deletion mutant of IR or to IGF-1R), inhibits insulin-induced internalization of IR, enhances insulin-stimulated glucose uptake, and competes with IRp for binding.	bind
3611	3	2202	6	10	NULL	0	NULL	IRp antibody	GP		does not bind					IGF-1R	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_21_11692_s_142	9326672	( iv) An antibody to IRp binds to IR (but not to a deletion mutant of IR or to IGF-1R), inhibits insulin-induced internalization of IR, enhances insulin-stimulated glucose uptake, and competes with IRp for binding.	bind
3612	4	2202	6	10	NULL	0	NULL	insulin	GP		induces					IR	GP	internalization of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_21_11692_s_142	9326672	( iv) An antibody to IRp binds to IR (but not to a deletion mutant of IR or to IGF-1R), inhibits insulin-induced internalization of IR, enhances insulin-stimulated glucose uptake, and competes with IRp for binding.	bind
3613	5	2202	6	10	NULL	0	NULL	IRp antibody	GP		inhibits					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_21_11692_s_142	9326672	( iv) An antibody to IRp binds to IR (but not to a deletion mutant of IR or to IGF-1R), inhibits insulin-induced internalization of IR, enhances insulin-stimulated glucose uptake, and competes with IRp for binding.	bind
3614	6	2202	6	10	NULL	0	NULL	insulin	GP		stimulates					glucose uptake	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_21_11692_s_142	9326672	( iv) An antibody to IRp binds to IR (but not to a deletion mutant of IR or to IGF-1R), inhibits insulin-induced internalization of IR, enhances insulin-stimulated glucose uptake, and competes with IRp for binding.	bind
3615	7	2202	6	10	NULL	0	NULL	IRp antibody	GP		enhances					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_21_11692_s_142	9326672	( iv) An antibody to IRp binds to IR (but not to a deletion mutant of IR or to IGF-1R), inhibits insulin-induced internalization of IR, enhances insulin-stimulated glucose uptake, and competes with IRp for binding.	bind
3616	8	2202	6	10	NULL	0	NULL	IRp	GP		bind					IR	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_21_11692_s_142	9326672	( iv) An antibody to IRp binds to IR (but not to a deletion mutant of IR or to IGF-1R), inhibits insulin-induced internalization of IR, enhances insulin-stimulated glucose uptake, and competes with IRp for binding.	bind
3617	9	2202	6	10	NULL	0	NULL	statement 1	Process		competes					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_21_11692_s_142	9326672	( iv) An antibody to IRp binds to IR (but not to a deletion mutant of IR or to IGF-1R), inhibits insulin-induced internalization of IR, enhances insulin-stimulated glucose uptake, and competes with IRp for binding.	bind
3775	1	2203	5	10	NULL	0	NULL	nuclear proteins	GP		bind					ks1	GP			cis regulatory elements	NULL	mutant reg-16	NULL	NULL	NULL	NULL	gw60_pnas_96_4_1445_s_197	9990043	( iv) In mutant reg-16, a high level of nuclear proteins binds to  ks1 cis regulatory elements (Fig.  6 B).	bind
3618	1	2203	6	10	NULL	0	NULL	nuclear proteins	GP		bind					ks1	GP			cis regulatory elements	NULL	mutant reg-16	NULL	NULL	NULL	NULL	gw60_pnas_96_4_1445_s_197	9990043	( iv) In mutant reg-16, a high level of nuclear proteins binds to  ks1 cis regulatory elements (Fig.  6 B).	bind
3776	1	2204	5	10	NULL	0	NULL	p300 histone acetyltransferase	GP		acetylate					core histones	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_genesdev_19_23_2912_s_122	16322561	( Left panel) Bacterially expressed NIR INHAT regions prevent acetylation of all core histones  by the p300 histone acetyltransferase in vitro.	bind
3777	2	2204	5	10	NULL	0	NULL	NIR INHAT	GP	bacterially expressed regions of	prevent					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_genesdev_19_23_2912_s_122	16322561	( Left panel) Bacterially expressed NIR INHAT regions prevent acetylation of all core histones  by the p300 histone acetyltransferase in vitro.	bind
3619	1	2204	6	10	NULL	0	NULL	histone acetyltransferase p300	GP		acetylates					core histones	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_genesdev_19_23_2912_s_122	16322561	( Left panel) Bacterially expressed NIR INHAT regions prevent acetylation of all core histones  by the p300 histone acetyltransferase in vitro.	bind
3620	2	2204	6	10	NULL	0	NULL	NIR INHAT	GP	Bacterially expressed regions of	prevents					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_genesdev_19_23_2912_s_122	16322561	( Left panel) Bacterially expressed NIR INHAT regions prevent acetylation of all core histones  by the p300 histone acetyltransferase in vitro.	bind
3778	1	2207	5	10	NULL	0	NULL	Nrp-1 receptors	GP		associate with		functionally			Plexin-signaling receptors	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_9_1013_s_76	15879551	( Left) Functional association of Nrp-1 and Nrp-2 receptors with Plexin-signaling receptors  transduce Sema3 signals.	bind
3779	2	2207	5	10	NULL	0	NULL	Nrp-2 receptors	GP		associate with		functionally			Plexin-signaling receptors	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_9_1013_s_76	15879551	( Left) Functional association of Nrp-1 and Nrp-2 receptors with Plexin-signaling receptors  transduce Sema3 signals.	bind
3780	3	2207	5	10	NULL	0	NULL	statement 1	Process		transduce					Sema3 signals	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_9_1013_s_76	15879551	( Left) Functional association of Nrp-1 and Nrp-2 receptors with Plexin-signaling receptors  transduce Sema3 signals.	bind
3781	4	2207	5	10	NULL	0	NULL	statement 2	Process		transduce					Sema3 signals	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_9_1013_s_76	15879551	( Left) Functional association of Nrp-1 and Nrp-2 receptors with Plexin-signaling receptors  transduce Sema3 signals.	bind
3621	1	2207	6	10	NULL	0	NULL	Nrp-1 receptor	GP		associate		functionaly			plexin-signaling receptors	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_9_1013_s_76	15879551	( Left) Functional association of Nrp-1 and Nrp-2 receptors with Plexin-signaling receptors  transduce Sema3 signals.	bind
3622	2	2207	6	10	NULL	0	NULL	Nrp-2 receptor	GP		associate		functionaly			plexin-signaling receptors	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_9_1013_s_76	15879551	( Left) Functional association of Nrp-1 and Nrp-2 receptors with Plexin-signaling receptors  transduce Sema3 signals.	bind
3623	3	2207	6	10	NULL	0	NULL	statement 1	Process		transduce					Sema3 signals	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_9_1013_s_76	15879551	( Left) Functional association of Nrp-1 and Nrp-2 receptors with Plexin-signaling receptors  transduce Sema3 signals.	bind
3624	4	2207	6	10	NULL	0	NULL	statement 2	Process		transduce					Sema3 signals	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_9_1013_s_76	15879551	( Left) Functional association of Nrp-1 and Nrp-2 receptors with Plexin-signaling receptors  transduce Sema3 signals.	bind
3782	1	2208	5	10	NULL	0	NULL	cGMP	Chemical		bind					monomeric PKG	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_5_2380_s_143	12591946	( Left) Model of cGMP binding to monomeric PKG that is used to generate binding curves.	bind
3625	1	2208	6	10	NULL	0	NULL	cGMP	Chemical		bind					monomeric PKG	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_5_2380_s_143	12591946	( Left) Model of cGMP binding to monomeric PKG that is used to generate binding curves.	bind
3783	1	2209	5	10	NULL	0	NULL	Cbl	GP		bind					IF	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevnutr_19_0_173_s_217	10448521	( Left) The transcytosis of Cbl following the apical internalization of Cbl bound to intrinsic  factor (IF).	bind
3784	2	2209	5	10	NULL	0	NULL	IF	GP		is					intrinsic factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevnutr_19_0_173_s_217	10448521	( Left) The transcytosis of Cbl following the apical internalization of Cbl bound to intrinsic  factor (IF).	bind
3785	3	2209	5	10	NULL	0	NULL	statement 1	Process		undergoes					apical internalization	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevnutr_19_0_173_s_217	10448521	( Left) The transcytosis of Cbl following the apical internalization of Cbl bound to intrinsic  factor (IF).	bind
3786	4	2209	5	10	NULL	0	NULL	statement 3	Process		leads to					Cbl	GP	transcytosis of			NULL		NULL	NULL	NULL	NULL	gw70_annurevnutr_19_0_173_s_217	10448521	( Left) The transcytosis of Cbl following the apical internalization of Cbl bound to intrinsic  factor (IF).	bind
3626	1	2209	6	10	NULL	0	NULL	Cbl	GP		bind					IF	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevnutr_19_0_173_s_217	10448521	( Left) The transcytosis of Cbl following the apical internalization of Cbl bound to intrinsic  factor (IF).	bind
3627	2	2209	6	10	NULL	0	NULL	IF	GP		is					intrinsic factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevnutr_19_0_173_s_217	10448521	( Left) The transcytosis of Cbl following the apical internalization of Cbl bound to intrinsic  factor (IF).	bind
46349	3	2209	6	10	NULL	0	NULL	statement 1	Process		undergoes					apical internalization	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevnutr_19_0_173_s_217	10448521	( Left) The transcytosis of Cbl following the apical internalization of Cbl bound to intrinsic  factor (IF).	bind
46351	4	2209	6	10	NULL	0	NULL	statement 3	Process		leads to					Cbl	GP	transcytosis of			NULL		NULL	NULL	NULL	NULL	gw70_annurevnutr_19_0_173_s_217	10448521	( Left) The transcytosis of Cbl following the apical internalization of Cbl bound to intrinsic  factor (IF).	bind
3788	1	2211	5	10	NULL	0	NULL	SRY	GP	wt	bind					DNA	NucleicAcid			SRY DNA-binding consesus site AACAAT	NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_12_7045_s_129	12764225	( Lower) A typical single EMSA experiment demonstrating SRYwt,  SRYR62G, and SRYR133W (860  pg) binding to the SRY DNA-binding consensus site  AACAAT.	bind
3789	2	2211	5	10	NULL	0	NULL	SRY	GP		bind			R62G		DNA	NucleicAcid			SRY DNA-binding consesus site AACAAT	NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_12_7045_s_129	12764225	( Lower) A typical single EMSA experiment demonstrating SRYwt,  SRYR62G, and SRYR133W (860  pg) binding to the SRY DNA-binding consensus site  AACAAT.	bind
3790	3	2211	5	10	NULL	0	NULL	SRY	GP		bind			R133W		DNA	NucleicAcid			SRY DNA-binding consesus site AACAAT	NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_12_7045_s_129	12764225	( Lower) A typical single EMSA experiment demonstrating SRYwt,  SRYR62G, and SRYR133W (860  pg) binding to the SRY DNA-binding consensus site  AACAAT.	bind
3628	1	2211	6	10	NULL	0	NULL	SRY	GP	wt	bind					DNA	NucleicAcid			SRY DNA-binding consensus site AACAAT	NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_12_7045_s_129	12764225	( Lower) A typical single EMSA experiment demonstrating SRYwt,  SRYR62G, and SRYR133W (860  pg) binding to the SRY DNA-binding consensus site  AACAAT.	bind
3629	2	2211	6	10	NULL	0	NULL	SRY	GP		bind			R62G		DNA	NucleicAcid			SRY DNA-binding consensus site AACAAT	NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_12_7045_s_129	12764225	( Lower) A typical single EMSA experiment demonstrating SRYwt,  SRYR62G, and SRYR133W (860  pg) binding to the SRY DNA-binding consensus site  AACAAT.	bind
3630	3	2211	6	10	NULL	0	NULL	SRY	GP		bind			R133W		DNA	NucleicAcid			SRY DNA-binding consensus site AACAAT	NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_12_7045_s_129	12764225	( Lower) A typical single EMSA experiment demonstrating SRYwt,  SRYR62G, and SRYR133W (860  pg) binding to the SRY DNA-binding consensus site  AACAAT.	bind
3791	1	2213	5	10	NULL	0	NULL	Go-GDP	GP		bind					MBP-Pins	GP	purified			NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_17_6524_s_108	16617104	( Lower) Go-GDP binds purified MBP-Pins; Go-GTP binds much less.	bind
3792	2	2213	5	10	NULL	0	NULL	Go-GTP	GP		bind		lesser			MBP-Pins	GP	purified			NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_17_6524_s_108	16617104	( Lower) Go-GDP binds purified MBP-Pins; Go-GTP binds much less.	bind
3631	1	2213	6	10	NULL	0	NULL	Go-GDP	GP		bind					MBP-Pins	GP	purified			NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_17_6524_s_108	16617104	( Lower) Go-GDP binds purified MBP-Pins; Go-GTP binds much less.	bind
3632	2	2213	6	10	NULL	0	NULL	Go-GTP	GP		bind		less			MBP-Pins	GP	purified			NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_17_6524_s_108	16617104	( Lower) Go-GDP binds purified MBP-Pins; Go-GTP binds much less.	bind
3793	1	2216	5	10	NULL	0	NULL	vitellogenin mRNA	NucleicAcid		contains				3''-UTR					two APyrUGA elements	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_23_12498_s_73	11050168	( Lower) The sequence of the vitellogenin B1 3''-UTR bound by vigilin containing the only two APyrUGA elements present in the 3''-UTR of vitellogenin mRNA ( 18).	bind
3794	2	2216	5	10	NULL	0	NULL	vitellogenin B1	NucleicAcid		bind				3''-UTR	vigilin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_23_12498_s_73	11050168	( Lower) The sequence of the vitellogenin B1 3''-UTR bound by vigilin containing the only two APyrUGA elements present in the 3''-UTR of vitellogenin mRNA ( 18).	bind
3633	1	2216	6	10	NULL	0	NULL	vitellogenin B1	NucleicAcid		bind				3''-UTR	vigilin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_23_12498_s_73	11050168	( Lower) The sequence of the vitellogenin B1 3''-UTR bound by vigilin containing the only two APyrUGA elements present in the 3''-UTR of vitellogenin mRNA ( 18).	bind
3634	2	2216	6	10	NULL	0	NULL	vitellogenin mRNA	NucleicAcid		contains				3''-UTR					two APyrUGA elements	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_23_12498_s_73	11050168	( Lower) The sequence of the vitellogenin B1 3''-UTR bound by vigilin containing the only two APyrUGA elements present in the 3''-UTR of vitellogenin mRNA ( 18).	bind
3811	1	2217	5	10	NULL	0	NULL				superimpose with			1-850		T3	GP	crystal structure			NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_12_7354_s_130	12777627	( Lower)1-850 superimposes with the crystal structure of T3  (green), bound to active TR  and clashes with the active conformation of helix  H12 (cyan).	bind
3812	2	2217	5	10	NULL	0	NULL				bind			1-850		TR	GP	active			NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_12_7354_s_130	12777627	( Lower)1-850 superimposes with the crystal structure of T3  (green), bound to active TR  and clashes with the active conformation of helix  H12 (cyan).	bind
3813	3	2217	5	10	NULL	0	NULL				clashes with			1-850		helix H12 	GP	active conformation of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_12_7354_s_130	12777627	( Lower)1-850 superimposes with the crystal structure of T3  (green), bound to active TR  and clashes with the active conformation of helix  H12 (cyan).	bind
4399	1	2217	6	10	NULL	0	NULL				superimpose with			1-850		T3	GP	crystal structure			NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_12_7354_s_130	12777627	( Lower)1-850 superimposes with the crystal structure of T3  (green), bound to active TR  and clashes with the active conformation of helix  H12 (cyan).	bind
4401	2	2217	6	10	NULL	0	NULL				bind			1-850		TR	GP	active			NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_12_7354_s_130	12777627	( Lower)1-850 superimposes with the crystal structure of T3  (green), bound to active TR  and clashes with the active conformation of helix  H12 (cyan).	bind
4404	3	2217	6	10	NULL	0	NULL				clashes with 			1-850		helix H12	GP	active conformation of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_12_7354_s_130	12777627	( Lower)1-850 superimposes with the crystal structure of T3  (green), bound to active TR  and clashes with the active conformation of helix  H12 (cyan).	bind
3814	1	2219	5	10	NULL	0	NULL	Shh	GP		induce					Gli1	GP	expression			NULL	dermal fibroblasts isolated from wild-type skin	NULL	NULL	NULL	NULL	gw60_genesdev_17_2_282_s_115	12533516	( M) Shh induces  Gli1 and  Ptc1 expression in dermal fibroblasts isolated from wild-type skin, as revealed by RT-PCR analysis.	bind
3815	2	2219	5	10	NULL	0	NULL	Shh	GP		induce					Ptc1	GP	expression			NULL	dermal fibroblasts isolated from wild-type skin	NULL	NULL	NULL	NULL	gw60_genesdev_17_2_282_s_115	12533516	( M) Shh induces  Gli1 and  Ptc1 expression in dermal fibroblasts isolated from wild-type skin, as revealed by RT-PCR analysis.	bind
3635	1	2219	6	10	NULL	0	NULL	Shh	GP		induces					Gli1	GP	expression of 			NULL	dermal fibroblasts isolated from wild-type skin	NULL	NULL	NULL	NULL	gw60_genesdev_17_2_282_s_115	12533516	( M) Shh induces  Gli1 and  Ptc1 expression in dermal fibroblasts isolated from wild-type skin, as revealed by RT-PCR analysis.	bind
3636	2	2219	6	10	NULL	0	NULL	Shh	GP		induces					Ptc1	GP	expression of 			NULL	dermal fibroblasts isolated from wild-type skin	NULL	NULL	NULL	NULL	gw60_genesdev_17_2_282_s_115	12533516	( M) Shh induces  Gli1 and  Ptc1 expression in dermal fibroblasts isolated from wild-type skin, as revealed by RT-PCR analysis.	bind
3816	1	2220	5	10	NULL	0	NULL	Hh	GP		bind					Ptc	GP				NULL	A-compartment cells near the A/P boundary (B cell) 	NULL	NULL	NULL	NULL	gw60_genesdev_16_18_2315_s_94	12231619	( Middle) In A-compartment cells near the A/P boundary (B cell) or cells near the MF (M cell), Hh binds Ptc, alleviating its repression on Smo.	bind
3817	2	2220	5	10	NULL	0	NULL	statement 1	Process		alleviate					Smo	GP	repression on			NULL	A-compartment cells near the A/P boundary (B cell)	NULL	NULL	NULL	NULL	gw60_genesdev_16_18_2315_s_94	12231619	( Middle) In A-compartment cells near the A/P boundary (B cell) or cells near the MF (M cell), Hh binds Ptc, alleviating its repression on Smo.	bind
52943	3	2220	5	10	NULL	0	NULL	Hh	GP		bind					Ptc	GP				NULL	cells near the MF (M cell)	NULL	NULL	NULL	NULL	gw60_genesdev_16_18_2315_s_94	12231619	( Middle) In A-compartment cells near the A/P boundary (B cell) or cells near the MF (M cell), Hh binds Ptc, alleviating its repression on Smo.	bind
52945	4	2220	5	10	NULL	0	NULL	statement 3	Process		alleviate					Smo	GP	repression on			NULL	cells near the MF (M cell)	NULL	NULL	NULL	NULL	gw60_genesdev_16_18_2315_s_94	12231619	( Middle) In A-compartment cells near the A/P boundary (B cell) or cells near the MF (M cell), Hh binds Ptc, alleviating its repression on Smo.	bind
3637	1	2220	6	10	NULL	0	NULL	Hh	GP		bind					Ptc	GP				NULL	In A-compartment cells near the A/P boundary (B cell) 	NULL	NULL	NULL	NULL	gw60_genesdev_16_18_2315_s_94	12231619	( Middle) In A-compartment cells near the A/P boundary (B cell) or cells near the MF (M cell), Hh binds Ptc, alleviating its repression on Smo.	bind
3638	2	2220	6	10	NULL	0	NULL	statement 1	Process		alleviate					Smo	GP	repression on			NULL	In A-compartment cells near the A/P boundary (B cell) 	NULL	NULL	NULL	NULL	gw60_genesdev_16_18_2315_s_94	12231619	( Middle) In A-compartment cells near the A/P boundary (B cell) or cells near the MF (M cell), Hh binds Ptc, alleviating its repression on Smo.	bind
52946	3	2220	6	10	NULL	0	NULL	Hh	GP		bind					Ptc	GP				NULL	cells near the MF (M cell)	NULL	NULL	NULL	NULL	gw60_genesdev_16_18_2315_s_94	12231619	( Middle) In A-compartment cells near the A/P boundary (B cell) or cells near the MF (M cell), Hh binds Ptc, alleviating its repression on Smo.	bind
52947	4	2220	6	10	NULL	0	NULL	statement 3	Process		alleviate					Smo	GP	repression on			NULL	cells near the MF (M cell)	NULL	NULL	NULL	NULL	gw60_genesdev_16_18_2315_s_94	12231619	( Middle) In A-compartment cells near the A/P boundary (B cell) or cells near the MF (M cell), Hh binds Ptc, alleviating its repression on Smo.	bind
3818	1	2221	5	10	NULL	0	NULL	III-31-C	Chemical		bind					PS1 NTF/CTF heterodimer	GP		active site		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_9_3230_s_160	15722417	( Middle) Transition-state analogue III-31-C binds to PS1 NTF/CTF heterodimer at the active  site, located internally and containing two aspartates (denoted as "`D"`).	bind
3819	2	2221	5	10	NULL	0	NULL	PS1 NTF/CTF heterodimer	GP		is located			active site		internally					NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_9_3230_s_160	15722417	( Middle) Transition-state analogue III-31-C binds to PS1 NTF/CTF heterodimer at the active  site, located internally and containing two aspartates (denoted as "`D"`).	bind
3820	3	2221	5	10	NULL	0	NULL	PS1 NTF/CTF heterodimer	GP		contains			active site		aspartate	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_9_3230_s_160	15722417	( Middle) Transition-state analogue III-31-C binds to PS1 NTF/CTF heterodimer at the active  site, located internally and containing two aspartates (denoted as "`D"`).	bind
46352	4	2221	5	10	NULL	0	NULL	III-31-C	Chemical		is a type of					Transition-state analogue	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_9_3230_s_160	15722417	( Middle) Transition-state analogue III-31-C binds to PS1 NTF/CTF heterodimer at the active  site, located internally and containing two aspartates (denoted as "`D"`).	bind
3710	1	2221	6	10	NULL	0	NULL	 III-31-C	Chemical		bind					PS1 NTF/CTF heterodimer	GP		active site		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_9_3230_s_160	15722417	( Middle) Transition-state analogue III-31-C binds to PS1 NTF/CTF heterodimer at the active  site, located internally and containing two aspartates (denoted as "`D"`).	bind
46353	2	2221	6	10	NULL	0	NULL	PS1 NTF/CTF heterodimer	GP		contains			active site		aspartate	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_9_3230_s_160	15722417	( Middle) Transition-state analogue III-31-C binds to PS1 NTF/CTF heterodimer at the active  site, located internally and containing two aspartates (denoted as "`D"`).	bind
46398	3	2221	6	10	NULL	0	NULL	III-31-C	Chemical		is a type of					Transition-state analogue	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_9_3230_s_160	15722417	( Middle) Transition-state analogue III-31-C binds to PS1 NTF/CTF heterodimer at the active  site, located internally and containing two aspartates (denoted as "`D"`).	bind
52948	4	2221	6	10	NULL	0	NULL	PS1 NTF/CTF heterodimer	Chemical		is located			active site		internally					NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_9_3230_s_160	15722417	( Middle) Transition-state analogue III-31-C binds to PS1 NTF/CTF heterodimer at the active  site, located internally and containing two aspartates (denoted as "`D"`).	bind
3821	1	2222	5	10	NULL	0	NULL	Lhx5	GP		bind					sfrp1a	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_development_133_16_3191_s_293	16854974	( O) Lhx5 binds to the  sfrp1a promoter.	bind
3711	1	2222	6	10	NULL	0	NULL	Lhx5	GP		bind					Sfrp1a	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_development_133_16_3191_s_293	16854974	( O) Lhx5 binds to the  sfrp1a promoter.	bind
3822	1	2223	5	10	NULL	0	NULL	lactoferrin	GP		bind					OVR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_31_18219_s_223	7543099	( Panel B), for lactoferrin binding to OVR ( Panel  C), and for binding of an unrelated single chain antibody to the  LDL receptor	bind
3823	2	2223	5	10	NULL	0	NULL	single chain antibody	GP	unrelated 	bind					 LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_31_18219_s_223	7543099	( Panel B), for lactoferrin binding to OVR ( Panel  C), and for binding of an unrelated single chain antibody to the  LDL receptor	bind
3712	1	2223	6	10	NULL	0	NULL	lactoferrin	GP		bind					OVR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_31_18219_s_223	7543099	( Panel B), for lactoferrin binding to OVR ( Panel  C), and for binding of an unrelated single chain antibody to the  LDL receptor	bind
3713	2	2223	6	10	NULL	0	NULL	single chain antibody	GP	unrelated	bind					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_31_18219_s_223	7543099	( Panel B), for lactoferrin binding to OVR ( Panel  C), and for binding of an unrelated single chain antibody to the  LDL receptor	bind
3824	1	2224	5	10	NULL	0	NULL	EGFR mAb 3A	GP		bind					Protein A	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_12_8335_s_107	10075741	( Panels A and  B) or EGFR mAbs 3A/4A bound to Protein A ( Panels C and  D), as described under	bind
5224	2	2224	5	10	NULL	0	NULL	EGFR mAb 4A	GP		bind					Protein A	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_12_8335_s_107	10075741	( Panels A and  B) or EGFR mAbs 3A/4A bound to Protein A ( Panels C and  D), as described under	bind
3714	1	2224	6	10	NULL	0	NULL	EGFR mAb 3A	GP		bind					Protein A	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_12_8335_s_107	10075741	( Panels A and  B) or EGFR mAbs 3A/4A bound to Protein A ( Panels C and  D), as described under	bind
3715	2	2224	6	10	NULL	0	NULL	EGFR mAb 4A	GP		bind					Protein A	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_12_8335_s_107	10075741	( Panels A and  B) or EGFR mAbs 3A/4A bound to Protein A ( Panels C and  D), as described under	bind
5251	1	2225	5	10	NULL	0	NULL	Epibatidine	Chemical		is a type of					nAChR agonist	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_287_3_847_s_2	9864263	( plus-or-minus )-Epibatidine (EPIB) and A-85380 are nicotinic acetylcholine receptor (nAChR) agonists that bind to the agonist ([3]cytisine) binding site with 40 to 50 pM affinity but have different affinities in nAChR subtype selective functional receptor assays.	bind
5252	2	2225	5	10	NULL	0	NULL	nAChR	GP		is					nicotinic acetylcholine receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_287_3_847_s_2	9864263	( plus-or-minus )-Epibatidine (EPIB) and A-85380 are nicotinic acetylcholine receptor (nAChR) agonists that bind to the agonist ([3]cytisine) binding site with 40 to 50 pM affinity but have different affinities in nAChR subtype selective functional receptor assays.	bind
5253	3	2225	5	10	NULL	0	NULL	Epibatidine	Chemical		bind					nAChR	GP		agonist (cytisine) binding site		NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_287_3_847_s_2	9864263	( plus-or-minus )-Epibatidine (EPIB) and A-85380 are nicotinic acetylcholine receptor (nAChR) agonists that bind to the agonist ([3]cytisine) binding site with 40 to 50 pM affinity but have different affinities in nAChR subtype selective functional receptor assays.	bind
5254	4	2225	5	10	NULL	0	NULL	A-85380	Chemical		is a type of					nAChR agonist	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_287_3_847_s_2	9864263	( plus-or-minus )-Epibatidine (EPIB) and A-85380 are nicotinic acetylcholine receptor (nAChR) agonists that bind to the agonist ([3]cytisine) binding site with 40 to 50 pM affinity but have different affinities in nAChR subtype selective functional receptor assays.	bind
5255	5	2225	5	10	NULL	0	NULL	A-85380	Chemical		bind					nAChR	GP		agonist (cytisine) binding site		NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_287_3_847_s_2	9864263	( plus-or-minus )-Epibatidine (EPIB) and A-85380 are nicotinic acetylcholine receptor (nAChR) agonists that bind to the agonist ([3]cytisine) binding site with 40 to 50 pM affinity but have different affinities in nAChR subtype selective functional receptor assays.	bind
46399	6	2225	5	10	NULL	0	NULL	EPIB	Chemical		is					Epibatidine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_287_3_847_s_2	9864263	( plus-or-minus )-Epibatidine (EPIB) and A-85380 are nicotinic acetylcholine receptor (nAChR) agonists that bind to the agonist ([3]cytisine) binding site with 40 to 50 pM affinity but have different affinities in nAChR subtype selective functional receptor assays.	bind
3925	1	2225	6	10	NULL	0	NULL	Epibatidine 	Chemical		is a type of					nAChR agonist	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_287_3_847_s_2	9864263	( plus-or-minus )-Epibatidine (EPIB) and A-85380 are nicotinic acetylcholine receptor (nAChR) agonists that bind to the agonist ([3]cytisine) binding site with 40 to 50 pM affinity but have different affinities in nAChR subtype selective functional receptor assays.	bind
3926	2	2225	6	10	NULL	0	NULL	A-85380	Chemical		is a type of					nAChR agonist	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_287_3_847_s_2	9864263	( plus-or-minus )-Epibatidine (EPIB) and A-85380 are nicotinic acetylcholine receptor (nAChR) agonists that bind to the agonist ([3]cytisine) binding site with 40 to 50 pM affinity but have different affinities in nAChR subtype selective functional receptor assays.	bind
3927	3	2225	6	10	NULL	0	NULL	nAChR	GP		is					nicotinic acetylcholine receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_287_3_847_s_2	9864263	( plus-or-minus )-Epibatidine (EPIB) and A-85380 are nicotinic acetylcholine receptor (nAChR) agonists that bind to the agonist ([3]cytisine) binding site with 40 to 50 pM affinity but have different affinities in nAChR subtype selective functional receptor assays.	bind
3928	4	2225	6	10	NULL	0	NULL	statement 1	Process		bind					nAChR	GP		agonist (cytisine) binding site		NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_287_3_847_s_2	9864263	( plus-or-minus )-Epibatidine (EPIB) and A-85380 are nicotinic acetylcholine receptor (nAChR) agonists that bind to the agonist ([3]cytisine) binding site with 40 to 50 pM affinity but have different affinities in nAChR subtype selective functional receptor assays.	bind
3929	5	2225	6	10	NULL	0	NULL	statement 2	Process		bind					nAChR	GP		agonist (cytisine) binding site		NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_287_3_847_s_2	9864263	( plus-or-minus )-Epibatidine (EPIB) and A-85380 are nicotinic acetylcholine receptor (nAChR) agonists that bind to the agonist ([3]cytisine) binding site with 40 to 50 pM affinity but have different affinities in nAChR subtype selective functional receptor assays.	bind
46400	6	2225	6	10	NULL	0	NULL	EPIB	Chemical		is					Epibatidine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_287_3_847_s_2	9864263	( plus-or-minus )-Epibatidine (EPIB) and A-85380 are nicotinic acetylcholine receptor (nAChR) agonists that bind to the agonist ([3]cytisine) binding site with 40 to 50 pM affinity but have different affinities in nAChR subtype selective functional receptor assays.	bind
3825	1	2226	5	10	NULL	0	NULL	tRNAs	NucleicAcid		bind					Arc1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_8_6000_s_111	11069915	( Pool A) contain tRNAs bound to Arc1p, whereas fractions 20-23	bind
3716	1	2226	6	10	NULL	0	NULL	tRNA	NucleicAcid		bind					Arc1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_8_6000_s_111	11069915	( Pool A) contain tRNAs bound to Arc1p, whereas fractions 20-23	bind
3826	1	2227	5	10	NULL	0	NULL	receptor for Activated- C Kinase 1	GP		bind		specifically			PKC	GP	activated			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_24_22073_s_36	11934885	( Receptor for  Activated- C  Kinase 1), specifically binds to activated PKC ( 24,  25).	bind
3717	1	2227	6	10	NULL	0	NULL	Receptor for Activated- C Kinase 1	GP		bind		specifically			PKC	GP	activated			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_24_22073_s_36	11934885	( Receptor for  Activated- C  Kinase 1), specifically binds to activated PKC ( 24,  25).	bind
3827	1	2228	5	10	NULL	0	NULL	Lz-AT	GP		is					Lz-binding site and adjacent AT sequences	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_7_838_s_108	12670867	( Right panel) A probe containing a Lz-binding site and adjacent AT sequences from the  dpn enhancer [Lz-AT(d1); Table  1] can bind Lz (black arrowhead, lane  9) and Cut (white arrowhead, lane  10).	bind
3828	2	2228	5	10	NULL	0	NULL	dpn	GP		bind				Lz-AT	Lz	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_7_838_s_108	12670867	( Right panel) A probe containing a Lz-binding site and adjacent AT sequences from the  dpn enhancer [Lz-AT(d1); Table  1] can bind Lz (black arrowhead, lane  9) and Cut (white arrowhead, lane  10).	bind
3829	3	2228	5	10	NULL	0	NULL	dpn	GP		bind				Lz-AT	Cut	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_7_838_s_108	12670867	( Right panel) A probe containing a Lz-binding site and adjacent AT sequences from the  dpn enhancer [Lz-AT(d1); Table  1] can bind Lz (black arrowhead, lane  9) and Cut (white arrowhead, lane  10).	bind
3718	1	2228	6	10	NULL	0	NULL	dpn	GP		bind				Lz-AT	Lz	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_7_838_s_108	12670867	( Right panel) A probe containing a Lz-binding site and adjacent AT sequences from the  dpn enhancer [Lz-AT(d1); Table  1] can bind Lz (black arrowhead, lane  9) and Cut (white arrowhead, lane  10).	bind
3930	2	2228	6	10	NULL	0	NULL	dpn	GP		bind				Lz-AT	Cut	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_7_838_s_108	12670867	( Right panel) A probe containing a Lz-binding site and adjacent AT sequences from the  dpn enhancer [Lz-AT(d1); Table  1] can bind Lz (black arrowhead, lane  9) and Cut (white arrowhead, lane  10).	bind
3960	3	2228	6	10	NULL	0	NULL	Lz-AT	GP		is					Lz-binding site and adjacent AT sequences	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_7_838_s_108	12670867	( Right panel) A probe containing a Lz-binding site and adjacent AT sequences from the  dpn enhancer [Lz-AT(d1); Table  1] can bind Lz (black arrowhead, lane  9) and Cut (white arrowhead, lane  10).	bind
3830	1	2229	5	10	NULL	0	NULL	immune complexes	GP		contains					G9a	GP				NULL	wild-type cells	NULL	NULL	NULL	NULL	gw70_genesdev_19_7_815_s_193	15774718	( Right panels) Similarly, immune complexes from wild-type cells obtained with anti-GLP antibody  also contain G9a.	bind
3719	1	2229	6	10	NULL	0	NULL	immune complex	GP		contain					G9a	GP				NULL	wild type cells	NULL	NULL	NULL	NULL	gw70_genesdev_19_7_815_s_193	15774718	( Right panels) Similarly, immune complexes from wild-type cells obtained with anti-GLP antibody  also contain G9a.	bind
3831	1	2230	5	10	NULL	0	NULL	Pax6	GP		is absent in				alpha enhancer	Vax1 DNA fragments	NucleicAcid				NULL	Vax double knock-outs	NULL	NULL	NULL	NULL	gw70_genesdev_19_10_1249_s_179	15905411	( Right panels) The Pax6 alpha-enhancer was not detected in Vax1 or Vax2 ChIP DNA fragments from  Vax double knock-outs, and Vax1 and Vax2 binding to the alpha-enhancer could not be detected in ChIPs performed from  Vax1 and  Vax2 mutants, respectively.	bind
3832	2	2230	5	10	NULL	0	NULL	Pax6	GP		is absent in				alpha enhancer	Vax2 DNA fragments	NucleicAcid				NULL	Vax double knock-outs	NULL	NULL	NULL	NULL	gw70_genesdev_19_10_1249_s_179	15905411	( Right panels) The Pax6 alpha-enhancer was not detected in Vax1 or Vax2 ChIP DNA fragments from  Vax double knock-outs, and Vax1 and Vax2 binding to the alpha-enhancer could not be detected in ChIPs performed from  Vax1 and  Vax2 mutants, respectively.	bind
3833	3	2230	5	10	NULL	0	NULL	Vax1	GP	mutant	does not bind					Pax6	GP			alpha enhancer	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_10_1249_s_179	15905411	( Right panels) The Pax6 alpha-enhancer was not detected in Vax1 or Vax2 ChIP DNA fragments from  Vax double knock-outs, and Vax1 and Vax2 binding to the alpha-enhancer could not be detected in ChIPs performed from  Vax1 and  Vax2 mutants, respectively.	bind
3834	4	2230	5	10	NULL	0	NULL	Vax2	GP	mutant	does not bind					Pax6	GP			alpha enhancer	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_10_1249_s_179	15905411	( Right panels) The Pax6 alpha-enhancer was not detected in Vax1 or Vax2 ChIP DNA fragments from  Vax double knock-outs, and Vax1 and Vax2 binding to the alpha-enhancer could not be detected in ChIPs performed from  Vax1 and  Vax2 mutants, respectively.	bind
3722	1	2230	6	10	NULL	0	NULL	Vax1	GP	mutant	does not bind					Pax6	GP			alpha-enhancer	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_10_1249_s_179	15905411	( Right panels) The Pax6 alpha-enhancer was not detected in Vax1 or Vax2 ChIP DNA fragments from  Vax double knock-outs, and Vax1 and Vax2 binding to the alpha-enhancer could not be detected in ChIPs performed from  Vax1 and  Vax2 mutants, respectively.	bind
3723	2	2230	6	10	NULL	0	NULL	Vax2	GP	mutant	does not bind					Pax6	GP			alpha-enhancer	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_10_1249_s_179	15905411	( Right panels) The Pax6 alpha-enhancer was not detected in Vax1 or Vax2 ChIP DNA fragments from  Vax double knock-outs, and Vax1 and Vax2 binding to the alpha-enhancer could not be detected in ChIPs performed from  Vax1 and  Vax2 mutants, respectively.	bind
5409	3	2230	6	10	NULL	0	NULL	Pax6	GP		is absent in				alpha enhancer	Vax 1 DNA fragments	NucleicAcid				NULL	Vax double knock-outs	NULL	NULL	NULL	NULL	gw70_genesdev_19_10_1249_s_179	15905411	( Right panels) The Pax6 alpha-enhancer was not detected in Vax1 or Vax2 ChIP DNA fragments from  Vax double knock-outs, and Vax1 and Vax2 binding to the alpha-enhancer could not be detected in ChIPs performed from  Vax1 and  Vax2 mutants, respectively.	bind
5410	4	2230	6	10	NULL	0	NULL	Pax6	GP		is absent in				alpha enhancer	Vax 2 DNA fragments	NucleicAcid				NULL	Vax double knock-outs	NULL	NULL	NULL	NULL	gw70_genesdev_19_10_1249_s_179	15905411	( Right panels) The Pax6 alpha-enhancer was not detected in Vax1 or Vax2 ChIP DNA fragments from  Vax double knock-outs, and Vax1 and Vax2 binding to the alpha-enhancer could not be detected in ChIPs performed from  Vax1 and  Vax2 mutants, respectively.	bind
4265	1	2232	5	10	NULL	0	NULL	E2F1	GP		bind					Bim	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_44_16090_s_153	16243973	( Right) E2F1 binding to the Bim promoter was analyzed by ChIP.	bind
3724	1	2232	6	10	NULL	0	NULL	E2F1	GP		bind					Bim	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_44_16090_s_153	16243973	( Right) E2F1 binding to the Bim promoter was analyzed by ChIP.	bind
3835	1	2233	5	10	NULL	0	NULL	SHBG	GP		bind					Te con	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_17_6740_s_79	15090645	( Right) Estimated free ( Upper) and SHBG-bound ( Lower) Te con.	bind
3725	1	2233	6	10	NULL	0	NULL	SHBG	GP		bind					Te con	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_17_6740_s_79	15090645	( Right) Estimated free ( Upper) and SHBG-bound ( Lower) Te con.	bind
4266	1	2234	5	10	NULL	0	NULL	alphaGMRx	GP		generate					H2O2	Chemical				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_102_14_5044_s_125	15795385	( Right) GM-dependent (100 nM) H2O2 generation  in vitro by alphaGMRx or mutant (C136Sx) bound to Ni+-nitrilotriacetic acid plates, as quantified by fluorescence spectroscopy.	bind
4267	2	2234	5	10	NULL	0	NULL			mutant	bind			C136Sx		Ni+-nitrilotriacetic acid plates	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_14_5044_s_125	15795385	( Right) GM-dependent (100 nM) H2O2 generation  in vitro by alphaGMRx or mutant (C136Sx) bound to Ni+-nitrilotriacetic acid plates, as quantified by fluorescence spectroscopy.	bind
46403	3	2234	5	10	NULL	0	NULL	statement 1	Process		is dependent on					GM	Cell				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_14_5044_s_125	15795385	( Right) GM-dependent (100 nM) H2O2 generation  in vitro by alphaGMRx or mutant (C136Sx) bound to Ni+-nitrilotriacetic acid plates, as quantified by fluorescence spectroscopy.	bind
3726	1	2234	6	10	NULL	0	NULL	alphaGMRx	GP		generates					H2O2	Chemical				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_102_14_5044_s_125	15795385	( Right) GM-dependent (100 nM) H2O2 generation  in vitro by alphaGMRx or mutant (C136Sx) bound to Ni+-nitrilotriacetic acid plates, as quantified by fluorescence spectroscopy.	bind
3727	2	2234	6	10	NULL	0	NULL	statement 1	Process		is dependent on					GM	Cell				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_14_5044_s_125	15795385	( Right) GM-dependent (100 nM) H2O2 generation  in vitro by alphaGMRx or mutant (C136Sx) bound to Ni+-nitrilotriacetic acid plates, as quantified by fluorescence spectroscopy.	bind
3728	3	2234	6	10	NULL	0	NULL			mutant	bind			C136Sx		Ni+-nitrilotriacetic acid plates	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_14_5044_s_125	15795385	( Right) GM-dependent (100 nM) H2O2 generation  in vitro by alphaGMRx or mutant (C136Sx) bound to Ni+-nitrilotriacetic acid plates, as quantified by fluorescence spectroscopy.	bind
3836	1	2235	5	10	NULL	0	NULL	Pg	GP		bind					mPR	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5619_594_s_18	12714732	( Right) In contrast, binding of Pg to mPR leads to inhibition of adenylyl cyclase through activation of Galphai or inhibition of Galphas.	bind
3837	2	2235	5	10	NULL	0	NULL	statement 1	Process		leads to					adenylyl cyclase	GP	inhibition of			NULL		NULL	NULL	NULL	NULL	gw60_science_300_5619_594_s_18	12714732	( Right) In contrast, binding of Pg to mPR leads to inhibition of adenylyl cyclase through activation of Galphai or inhibition of Galphas.	bind
3838	3	2235	5	10	NULL	0	NULL	statement 2	Process		occurs through					Galphai	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_science_300_5619_594_s_18	12714732	( Right) In contrast, binding of Pg to mPR leads to inhibition of adenylyl cyclase through activation of Galphai or inhibition of Galphas.	bind
3839	4	2235	5	10	NULL	0	NULL	statement 2	Process		occurs through					Galphas	GP	inhibition of			NULL		NULL	NULL	NULL	NULL	gw60_science_300_5619_594_s_18	12714732	( Right) In contrast, binding of Pg to mPR leads to inhibition of adenylyl cyclase through activation of Galphai or inhibition of Galphas.	bind
5225	5	2235	5	10	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5619_594_s_18	12714732	( Right) In contrast, binding of Pg to mPR leads to inhibition of adenylyl cyclase through activation of Galphai or inhibition of Galphas.	bind
3729	1	2235	6	10	NULL	0	NULL	Pg	GP		bind					mPR	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5619_594_s_18	12714732	( Right) In contrast, binding of Pg to mPR leads to inhibition of adenylyl cyclase through activation of Galphai or inhibition of Galphas.	bind
3730	2	2235	6	10	NULL	0	NULL	statement 1	Process		leads to					adenylyl cyclase	GP	inhibition of			NULL		NULL	NULL	NULL	NULL	gw60_science_300_5619_594_s_18	12714732	( Right) In contrast, binding of Pg to mPR leads to inhibition of adenylyl cyclase through activation of Galphai or inhibition of Galphas.	bind
3731	3	2235	6	10	NULL	0	NULL	statement 1	Process		leads to					Galphai	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_science_300_5619_594_s_18	12714732	( Right) In contrast, binding of Pg to mPR leads to inhibition of adenylyl cyclase through activation of Galphai or inhibition of Galphas.	bind
3732	4	2235	6	10	NULL	0	NULL	statement 1	Process		leads to					Galphas	GP	inhibition of			NULL		NULL	NULL	NULL	NULL	gw60_science_300_5619_594_s_18	12714732	( Right) In contrast, binding of Pg to mPR leads to inhibition of adenylyl cyclase through activation of Galphai or inhibition of Galphas.	bind
4861	5	2235	6	10	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5619_594_s_18	12714732	( Right) In contrast, binding of Pg to mPR leads to inhibition of adenylyl cyclase through activation of Galphai or inhibition of Galphas.	bind
3857	1	2236	5	10	NULL	0	NULL	VCB	GP		bind			 pVHL		Elongin B/C complex	GP		Socs box		NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_70_0_503_s_430	11395416	( Right) In VCB, the substrate-recognizing subunit pVHL binds to the Elongin B/C complex  through a motif known as the Socs box, which is present in other proteins that may  be the substrate-recognizing subunits of distinct VCB-like E3s ( 31,  139).	bind
3858	2	2236	5	10	NULL	0	NULL				is present in			Socs box		VCB-like E3s	GP		substrate-recognizing subunits of 		NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_70_0_503_s_430	11395416	( Right) In VCB, the substrate-recognizing subunit pVHL binds to the Elongin B/C complex  through a motif known as the Socs box, which is present in other proteins that may  be the substrate-recognizing subunits of distinct VCB-like E3s ( 31,  139).	bind
46405	3	2236	5	10	NULL	0	NULL	pVHL	GP		is a type of					substrate-recognizing subunit	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_70_0_503_s_430	11395416	( Right) In VCB, the substrate-recognizing subunit pVHL binds to the Elongin B/C complex  through a motif known as the Socs box, which is present in other proteins that may  be the substrate-recognizing subunits of distinct VCB-like E3s ( 31,  139).	bind
3733	1	2236	6	10	NULL	0	NULL	VCB	GP		bind			pVHL		Elongin B/C complex	GP		Socs box		NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_70_0_503_s_430	11395416	( Right) In VCB, the substrate-recognizing subunit pVHL binds to the Elongin B/C complex  through a motif known as the Socs box, which is present in other proteins that may  be the substrate-recognizing subunits of distinct VCB-like E3s ( 31,  139).	bind
4862	2	2236	6	10	NULL	0	NULL				is present in			Socs box		VCB-like E3s	GP		substrate-recognizing subunits of		NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_70_0_503_s_430	11395416	( Right) In VCB, the substrate-recognizing subunit pVHL binds to the Elongin B/C complex  through a motif known as the Socs box, which is present in other proteins that may  be the substrate-recognizing subunits of distinct VCB-like E3s ( 31,  139).	bind
46406	3	2236	6	10	NULL	0	NULL	pVHL	GP		is a type of					substrate-recognizing subunit	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_70_0_503_s_430	11395416	( Right) In VCB, the substrate-recognizing subunit pVHL binds to the Elongin B/C complex  through a motif known as the Socs box, which is present in other proteins that may  be the substrate-recognizing subunits of distinct VCB-like E3s ( 31,  139).	bind
3859	1	2237	5	10	NULL	0	NULL	EAC3d	GP		bind					CD21	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_16_10641_s_192	12122212	( Right) Photomicrographs (magnification x137) showing EAC3d binding to CD21 and CD21mut, but not to L cells transfected with vector alone.	bind
3860	2	2237	5	10	NULL	0	NULL	EAC3d	GP		bind					CD21	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_16_10641_s_192	12122212	( Right) Photomicrographs (magnification x137) showing EAC3d binding to CD21 and CD21mut, but not to L cells transfected with vector alone.	bind
3861	3	2237	5	10	NULL	0	NULL	EAC3d	GP		does not bind					L cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_16_10641_s_192	12122212	( Right) Photomicrographs (magnification x137) showing EAC3d binding to CD21 and CD21mut, but not to L cells transfected with vector alone.	bind
3734	1	2237	6	10	NULL	0	NULL	EAC3d	GP		bind					CD21	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_16_10641_s_192	12122212	( Right) Photomicrographs (magnification x137) showing EAC3d binding to CD21 and CD21mut, but not to L cells transfected with vector alone.	bind
3735	2	2237	6	10	NULL	0	NULL	EAC3d	GP		bind					CD21	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_16_10641_s_192	12122212	( Right) Photomicrographs (magnification x137) showing EAC3d binding to CD21 and CD21mut, but not to L cells transfected with vector alone.	bind
3736	3	2237	6	10	NULL	0	NULL	EAC3d	GP		does not bind					L cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_16_10641_s_192	12122212	( Right) Photomicrographs (magnification x137) showing EAC3d binding to CD21 and CD21mut, but not to L cells transfected with vector alone.	bind
3862	1	2238	5	10	NULL	0	NULL	fMTX	Chemical		bind		high-affinity			DHFR	GP	reconstituted			NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_10_5394_s_91	10318894	( Right) The fluorescence assay is based on high-affinity binding of the specific DHFR inhibitor fMTX to reconstituted DHFR.	bind
46407	2	2238	5	10	NULL	0	NULL	fMTX	Chemical		is a type of					DHFR inhibitor	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_10_5394_s_91	10318894	( Right) The fluorescence assay is based on high-affinity binding of the specific DHFR inhibitor fMTX to reconstituted DHFR.	bind
3803	1	2238	6	10	NULL	0	NULL	fMTX	Chemical		bind		high affinity			DHFR	GP	reconstituted			NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_10_5394_s_91	10318894	( Right) The fluorescence assay is based on high-affinity binding of the specific DHFR inhibitor fMTX to reconstituted DHFR.	bind
46408	2	2238	6	10	NULL	0	NULL	fMTX	Chemical		is a type of					DHFR inhibitor	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_10_5394_s_91	10318894	( Right) The fluorescence assay is based on high-affinity binding of the specific DHFR inhibitor fMTX to reconstituted DHFR.	bind
3864	1	2239	5	10	NULL	0	NULL	HsUbc2b	GP		bind					Uba1	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26823_s_210	12740388	( Table  II) is in the range of the  K m values  of 123  plus-or-minus  19 and 102  plus-or-minus  13 nM found for HsUbc2b binding  to human and rabbit Uba1 orthologs, respectively  ( ).	bind
3866	2	2239	5	10	NULL	0	NULL	HsUbc2b	GP		bind					Uba1	GP	rabbit			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26823_s_210	12740388	( Table  II) is in the range of the  K m values  of 123  plus-or-minus  19 and 102  plus-or-minus  13 nM found for HsUbc2b binding  to human and rabbit Uba1 orthologs, respectively  ( ).	bind
3805	1	2239	6	10	NULL	0	NULL	HsUbc2b	GP		bind					Uba1	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26823_s_210	12740388	( Table  II) is in the range of the  K m values  of 123  plus-or-minus  19 and 102  plus-or-minus  13 nM found for HsUbc2b binding  to human and rabbit Uba1 orthologs, respectively  ( ).	bind
3806	2	2239	6	10	NULL	0	NULL	HsUbc2b	GP		bind					Uba1	GP	rabbit			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26823_s_210	12740388	( Table  II) is in the range of the  K m values  of 123  plus-or-minus  19 and 102  plus-or-minus  13 nM found for HsUbc2b binding  to human and rabbit Uba1 orthologs, respectively  ( ).	bind
3869	1	2240	5	10	NULL	0	NULL	ATP	Chemical		bind					Uba1	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26823_s_208	12740388	( Table  II) was considerably higher than the   K m of 7.0  plus-or-minus  1.1 muM recently  reported for ATP binding to human Uba1  ( ); however, Nedd8  activation must remain saturating with respect to the normal cellular ATP  concentration of about 5 mM.	bind
3807	1	2240	6	10	NULL	0	NULL	ATP	Chemical		bind					Uba1	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26823_s_208	12740388	( Table  II) was considerably higher than the   K m of 7.0  plus-or-minus  1.1 muM recently  reported for ATP binding to human Uba1  ( ); however, Nedd8  activation must remain saturating with respect to the normal cellular ATP  concentration of about 5 mM.	bind
3873	1	2242	5	10	NULL	0	NULL	Nedd4	GP		bind					ENaC	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_20019_s_217	12654927	( Table  II), suggesting that the inhibitory role of intracellular  Na+ is not mediated by directly affecting the binding of Nedd4 to  ENaC.	bind
3874	2	2242	5	10	NULL	0	NULL	Na+	Chemical	inhibitory role of;;intracellular	is not mediated by					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_20019_s_217	12654927	( Table  II), suggesting that the inhibitory role of intracellular  Na+ is not mediated by directly affecting the binding of Nedd4 to  ENaC.	bind
3840	1	2242	6	10	NULL	0	NULL	Nedd4	GP		bind					ENaC	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_20019_s_217	12654927	( Table  II), suggesting that the inhibitory role of intracellular  Na+ is not mediated by directly affecting the binding of Nedd4 to  ENaC.	bind
3841	2	2242	6	10	NULL	0	NULL	Na+	Chemical	inhibitory role of;; intracellular	is not mediated by					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_20019_s_217	12654927	( Table  II), suggesting that the inhibitory role of intracellular  Na+ is not mediated by directly affecting the binding of Nedd4 to  ENaC.	bind
3875	1	2243	5	10	NULL	0	NULL	ATP	Chemical		bind					NBD1	GP	mutant	C682A		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_33_30764_s_184	12783859	( Table  II, 9.0  versus 8.5), further supporting our conclusion  that the  K d value was mainly attributed to ATP  binding to the C682A-mutated NBD1.	bind
3842	1	2243	6	10	NULL	0	NULL	ATP	Chemical		bind					NBD1	GP	mutant	 C682A		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_33_30764_s_184	12783859	( Table  II, 9.0  versus 8.5), further supporting our conclusion  that the  K d value was mainly attributed to ATP  binding to the C682A-mutated NBD1.	bind
3877	1	2244	5	10	NULL	0	NULL	sgk1	GP		does not bind					Nedd4-2	GP		WW domains		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_20019_s_223	12654927	( Table  III), suggesting that sgk1 does not bind (or binds very poorly) to  the WW domains of Nedd4-2.	bind
3878	2	2244	5	10	NULL	0	NULL	sgk1	GP		bind		very poorly			Nedd4-2	GP		WW domains		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_20019_s_223	12654927	( Table  III), suggesting that sgk1 does not bind (or binds very poorly) to  the WW domains of Nedd4-2.	bind
46409	3	2244	5	10	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_20019_s_223	12654927	( Table  III), suggesting that sgk1 does not bind (or binds very poorly) to  the WW domains of Nedd4-2.	bind
3843	1	2244	6	10	NULL	0	NULL	sgk1	GP		does not bind					Nedd4-2	GP		WW domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_20019_s_223	12654927	( Table  III), suggesting that sgk1 does not bind (or binds very poorly) to  the WW domains of Nedd4-2.	bind
3844	2	2244	6	10	NULL	0	NULL	sgk1	GP		bind		very poorly			Nedd4-2	GP		WW domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_20019_s_223	12654927	( Table  III), suggesting that sgk1 does not bind (or binds very poorly) to  the WW domains of Nedd4-2.	bind
46410	3	2244	6	10	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_20019_s_223	12654927	( Table  III), suggesting that sgk1 does not bind (or binds very poorly) to  the WW domains of Nedd4-2.	bind
3879	1	2245	5	10	NULL	0	NULL	PAI-1	GP		bind		low affinity			LRP	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_21_22595_s_318	15001579	( Table I) and others ( - ) have shown that these forms of PAI-1 only bind to LRP with low affinity.	bind
3845	1	2245	6	10	NULL	0	NULL	PAI-1	GP		bind		low affinity			LRP	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_21_22595_s_318	15001579	( Table I) and others ( - ) have shown that these forms of PAI-1 only bind to LRP with low affinity.	bind
3880	1	2246	5	10	NULL	0	NULL	Rabaptin-5	GP		does not bind		directly			ubiquitin	GP				NULL	cytosol	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_30_31409_s_258	15143060	( Table I), it is likely to derive from the presence in the cytosol of Rabaptin-5-associated proteins that also bind ubiquitin or undergo ubiquitin-dependent modification (Rabaptin-5 does not bind ubiquitin directly; results not shown).	bind
3881	2	2246	5	10	NULL	0	NULL	Rabaptin-5-associated proteins	GP		bind					ubiquitin	GP				NULL	cytosol	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_30_31409_s_258	15143060	( Table I), it is likely to derive from the presence in the cytosol of Rabaptin-5-associated proteins that also bind ubiquitin or undergo ubiquitin-dependent modification (Rabaptin-5 does not bind ubiquitin directly; results not shown).	bind
3882	3	2246	5	10	NULL	0	NULL	Rabaptin-5-associated proteins	GP		undergoes					ubiquitin-dependent modification	Process				NULL	cytosol	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_30_31409_s_258	15143060	( Table I), it is likely to derive from the presence in the cytosol of Rabaptin-5-associated proteins that also bind ubiquitin or undergo ubiquitin-dependent modification (Rabaptin-5 does not bind ubiquitin directly; results not shown).	bind
3846	1	2246	6	10	NULL	0	NULL	Rabaptin-5-associated proteins	GP		bind					ubiquitin	GP				NULL	cytosol	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_30_31409_s_258	15143060	( Table I), it is likely to derive from the presence in the cytosol of Rabaptin-5-associated proteins that also bind ubiquitin or undergo ubiquitin-dependent modification (Rabaptin-5 does not bind ubiquitin directly; results not shown).	bind
3847	2	2246	6	10	NULL	0	NULL	Rabaptin-5-associated proteins	GP		undergoes					ubiquitin-dependent modification	Process				NULL	cytosol	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_30_31409_s_258	15143060	( Table I), it is likely to derive from the presence in the cytosol of Rabaptin-5-associated proteins that also bind ubiquitin or undergo ubiquitin-dependent modification (Rabaptin-5 does not bind ubiquitin directly; results not shown).	bind
3848	3	2246	6	10	NULL	0	NULL	Rabaptin-5	GP		does not bind		directly			ubiquitin	GP				NULL	cytosol	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_30_31409_s_258	15143060	( Table I), it is likely to derive from the presence in the cytosol of Rabaptin-5-associated proteins that also bind ubiquitin or undergo ubiquitin-dependent modification (Rabaptin-5 does not bind ubiquitin directly; results not shown).	bind
3883	1	2247	5	10	NULL	0	NULL	Sti1	GP		bind		weakly			Ssa1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_28_25970_s_144	12716905	( Table I), Sti1 binding to Ssa1  is about 2 orders of magnitude weakerR.	bind
3849	1	2247	6	10	NULL	0	NULL	Sti1	GP		bind		weakly			Ssa1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_28_25970_s_144	12716905	( Table I), Sti1 binding to Ssa1  is about 2 orders of magnitude weakerR.	bind
3931	1	2248	5	10	NULL	0	NULL	dGTP	Chemical		is incorporated into					primer strand	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_17_2957_s_84	16107880	( Table I), we found that dGTP was incorporated into the primer strand and that the product  PPi remains bound to Dpo4 and occupies the same space as the triphosphate moiety  of dNTP ( Figure 1D).	bind
3932	2	2248	5	10	NULL	0	NULL	PPi	Chemical		bind					Dpo4	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_17_2957_s_84	16107880	( Table I), we found that dGTP was incorporated into the primer strand and that the product  PPi remains bound to Dpo4 and occupies the same space as the triphosphate moiety  of dNTP ( Figure 1D).	bind
3850	1	2248	6	10	NULL	0	NULL	PPi	Chemical		bind					Dpo4	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_17_2957_s_84	16107880	( Table I), we found that dGTP was incorporated into the primer strand and that the product  PPi remains bound to Dpo4 and occupies the same space as the triphosphate moiety  of dNTP ( Figure 1D).	bind
3851	2	2248	6	10	NULL	0	NULL	dGTP	Chemical		incorporates					primer strand	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_17_2957_s_84	16107880	( Table I), we found that dGTP was incorporated into the primer strand and that the product  PPi remains bound to Dpo4 and occupies the same space as the triphosphate moiety  of dNTP ( Figure 1D).	bind
3934	1	2251	5	10	NULL	0	NULL	apoA-I	GP	WT	bind					ABCA1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_48_49931_s_242	15383537	( Table II) and the  Kd value for binding of WT apoA-I to ABCA1 is 2 mug/ml ( ).	bind
3852	1	2251	6	10	NULL	0	NULL	apoA-I	GP	wild type	bind					ABCA1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_48_49931_s_242	15383537	( Table II) and the  Kd value for binding of WT apoA-I to ABCA1 is 2 mug/ml ( ).	bind
3977	1	2252	5	10	NULL	0	NULL				does not bind		stoichiometrically	R281A		oriC	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_49_51156_s_217	15371441	( Table II) revealed that R281A fails to bind stoichiometrically to  oriC, in contrast to gel mobility shift assays in which the mutant DnaA was comparable with wild-type DnaA in binding to the DnaA boxes of  oriC ( Fig. 3).	bind
3978	2	2252	5	10	NULL	0	NULL	DnaA	GP	wild-type	bind					oriC	NucleicAcid			DnaA boxes	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_49_51156_s_217	15371441	( Table II) revealed that R281A fails to bind stoichiometrically to  oriC, in contrast to gel mobility shift assays in which the mutant DnaA was comparable with wild-type DnaA in binding to the DnaA boxes of  oriC ( Fig. 3).	bind
4260	3	2252	5	10	NULL	0	NULL	DnaA	GP	mutant	bind					oriC	NucleicAcid			DnaA boxes	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_49_51156_s_217	15371441	( Table II) revealed that R281A fails to bind stoichiometrically to  oriC, in contrast to gel mobility shift assays in which the mutant DnaA was comparable with wild-type DnaA in binding to the DnaA boxes of  oriC ( Fig. 3).	bind
3853	1	2252	6	10	NULL	0	NULL	DnaA	GP	wild type	bind					oriC	NucleicAcid			DnaA boxes	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_49_51156_s_217	15371441	( Table II) revealed that R281A fails to bind stoichiometrically to  oriC, in contrast to gel mobility shift assays in which the mutant DnaA was comparable with wild-type DnaA in binding to the DnaA boxes of  oriC ( Fig. 3).	bind
3854	2	2252	6	10	NULL	0	NULL	DnaA	GP	mutant	bind					oriC	NucleicAcid			DnaA boxes	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_49_51156_s_217	15371441	( Table II) revealed that R281A fails to bind stoichiometrically to  oriC, in contrast to gel mobility shift assays in which the mutant DnaA was comparable with wild-type DnaA in binding to the DnaA boxes of  oriC ( Fig. 3).	bind
3855	3	2252	6	10	NULL	0	NULL				does not bind		stoichiometrically	 R281A		oriC	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_49_51156_s_217	15371441	( Table II) revealed that R281A fails to bind stoichiometrically to  oriC, in contrast to gel mobility shift assays in which the mutant DnaA was comparable with wild-type DnaA in binding to the DnaA boxes of  oriC ( Fig. 3).	bind
3980	1	2253	5	10	NULL	0	NULL	Runx2	GP		bind					osteocalcin	GP			cis-acting elements in promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_19_20307_s_159	15007057	( Table II) was not sufficient to normalize  Runx2 binding to  cis-acting elements in the osteocalcin promoter ( Fig. 5 C).	bind
3856	1	2253	6	10	NULL	0	NULL	Runx2 	GP		bind					osteocalcin	GP			cis-acting element of promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_19_20307_s_159	15007057	( Table II) was not sufficient to normalize  Runx2 binding to  cis-acting elements in the osteocalcin promoter ( Fig. 5 C).	bind
3981	1	2254	5	10	NULL	0	NULL				bind			L2 loop		BlaR1	GP		sensor domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_45_47278_s_265	15322076	( Table II), perhaps because either tag interferes with the binding of the L2 loop to the BlaR1 sensor domain.	bind
3863	1	2254	6	10	NULL	0	NULL				bind			L2 loop		BlaR1	GP		sensor domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_45_47278_s_265	15322076	( Table II), perhaps because either tag interferes with the binding of the L2 loop to the BlaR1 sensor domain.	bind
3983	1	2255	5	10	NULL	0	NULL	LT	GP		bind					bacteria	Organism	Re mutant			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_8070_s_82	14660669	( Table II), purified Re LPS would be able to block the binding of LT to Re mutant bacteria.	bind
3984	2	2255	5	10	NULL	0	NULL	Re LPS	Chemical	purified	block					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_8070_s_82	14660669	( Table II), purified Re LPS would be able to block the binding of LT to Re mutant bacteria.	bind
3865	1	2255	6	10	NULL	0	NULL	LT	GP		bind					bacteria	Organism	Re mutant			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_8070_s_82	14660669	( Table II), purified Re LPS would be able to block the binding of LT to Re mutant bacteria.	bind
3867	2	2255	6	10	NULL	0	NULL	Re LPS	Chemical	purified	blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_8070_s_82	14660669	( Table II), purified Re LPS would be able to block the binding of LT to Re mutant bacteria.	bind
3985	1	2256	5	10	NULL	0	NULL	galectin-4	GP		bind					glycosphingolipids	Chemical	sulfated			NULL	gastrointestinal tract	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_6_4730_s_220	15546874	( Table II), the binding between galectin-4 and sulfated glycosphingolipids may function for the cell adhesion of epithelial cells in the gastrointestinal tract.	bind
3986	2	2256	5	10	NULL	0	NULL	statement 1	Process		function for		may			epithelial cells	Cell	cell adhesion of			NULL	gastrointestinal tract	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_6_4730_s_220	15546874	( Table II), the binding between galectin-4 and sulfated glycosphingolipids may function for the cell adhesion of epithelial cells in the gastrointestinal tract.	bind
3868	1	2256	6	10	NULL	0	NULL	galectin-4	GP		bind					glycosphingolipids	Chemical	sulfated			NULL	gastrointestinal tract	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_6_4730_s_220	15546874	( Table II), the binding between galectin-4 and sulfated glycosphingolipids may function for the cell adhesion of epithelial cells in the gastrointestinal tract.	bind
3870	2	2256	6	10	NULL	0	NULL	statement 1	Process		may act in					epithelial cells	Cell	cell adhesion of			NULL	gastrointestinal tract	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_6_4730_s_220	15546874	( Table II), the binding between galectin-4 and sulfated glycosphingolipids may function for the cell adhesion of epithelial cells in the gastrointestinal tract.	bind
3987	1	2257	5	10	NULL	0	NULL	cGMP	Chemical		bind					PDE2A GAF-AB	GP		GAF-B domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_36_37928_s_188	15210692	( Table II), which is consistent with the crystal structure that showed cGMP bound to only the GAF-B domain of PDE2A GAF-AB ( ).	bind
3871	1	2257	6	10	NULL	0	NULL	cGMP	Chemical		bind					PDE2A  GAF-AB	GP		GAF-B domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_36_37928_s_188	15210692	( Table II), which is consistent with the crystal structure that showed cGMP bound to only the GAF-B domain of PDE2A GAF-AB ( ).	bind
3988	1	2261	5	10	NULL	0	NULL	Sp1	GP		bind					DNA	NucleicAcid			GC boxes in cellular promoters	NULL		NULL	NULL	NULL	NULL	gw60_science_296_5576_2149_s_19	12077389	( Top) The transcription factor Sp1 binds to DNA elements called GC boxes in cellular promoters.	bind
52989	2	2261	5	10	NULL	0	NULL	Sp1	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_296_5576_2149_s_19	12077389	( Top) The transcription factor Sp1 binds to DNA elements called GC boxes in cellular promoters.	bind
3884	1	2261	6	10	NULL	0	NULL	Sp1	GP		bind					DNA	NucleicAcid			GC box in cellular promoter	NULL		NULL	NULL	NULL	NULL	gw60_science_296_5576_2149_s_19	12077389	( Top) The transcription factor Sp1 binds to DNA elements called GC boxes in cellular promoters.	bind
52990	2	2261	6	10	NULL	0	NULL	Sp1	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_296_5576_2149_s_19	12077389	( Top) The transcription factor Sp1 binds to DNA elements called GC boxes in cellular promoters.	bind
3989	1	2264	5	10	NULL	0	NULL	mSin3a	GP		bind					KLF11	GP	Flag-tagged;; WT			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_13_4807_s_117	15774581	( Upper) A representative Western blot of coimmunoprecipitation experiments ( n = 2) showing mSin3a binding of Flag-tagged KLF11 (WT and variants) or empty vector  (control).	bind
3990	2	2264	5	10	NULL	0	NULL	mSin3a	GP		bind					KLF11	GP	Flag-tagged ;;variants			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_13_4807_s_117	15774581	( Upper) A representative Western blot of coimmunoprecipitation experiments ( n = 2) showing mSin3a binding of Flag-tagged KLF11 (WT and variants) or empty vector  (control).	bind
3885	1	2264	6	10	NULL	0	NULL	mSin3a	GP		bind					KLF11	GP	 Flag-tagged ;; wild type			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_13_4807_s_117	15774581	( Upper) A representative Western blot of coimmunoprecipitation experiments ( n = 2) showing mSin3a binding of Flag-tagged KLF11 (WT and variants) or empty vector  (control).	bind
3886	2	2264	6	10	NULL	0	NULL	mSin3a	GP		bind					KLF11	GP	 Flag-tagged;; variant			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_13_4807_s_117	15774581	( Upper) A representative Western blot of coimmunoprecipitation experiments ( n = 2) showing mSin3a binding of Flag-tagged KLF11 (WT and variants) or empty vector  (control).	bind
3992	1	2266	5	10	NULL	0	NULL	 GAS1 expressing cells	Cell		does not bind					IgG	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_20_11347_s_85	11572986	( Upper) Cells expressing GAS1 (red, detected by anti-GAS1 and Cy3-2 degrees  Abs) do not bind human IgG (Ig, green, detected by FITC-anti-Fc).	bind
3888	1	2266	6	10	NULL	0	NULL	GAS1 expressing cells	Cell		does not bind					IgG	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_20_11347_s_85	11572986	( Upper) Cells expressing GAS1 (red, detected by anti-GAS1 and Cy3-2 degrees  Abs) do not bind human IgG (Ig, green, detected by FITC-anti-Fc).	bind
3993	1	2267	5	10	NULL	0	NULL	Crk	GP		bind			SH2 domain		Crk phosphopeptide	GP		residues 221-224		NULL	in the ternary complex	NULL	NULL	NULL	NULL	gw60_pnas_99_22_14053_s_136	12384576	( Upper) Detail of the Crk SH2 domain bound to the Crk phosphopeptide (residues 221-224) in the ternary complex.	bind
3889	1	2267	6	10	NULL	0	NULL	Crk	GP		bind			SH2 domain		Crk phosphopeptide 	GP		residues 221-224		NULL	ternary complex	NULL	NULL	NULL	NULL	gw60_pnas_99_22_14053_s_136	12384576	( Upper) Detail of the Crk SH2 domain bound to the Crk phosphopeptide (residues 221-224) in the ternary complex.	bind
3994	1	2268	5	10	NULL	0	NULL	epsins	GP	yeast	bind					Cdc24	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_11_4116_s_211	16537494	( vii) Other authors  and our unpublished data show that the yeast epsins bind Cdc24, the Cdc42 guanine nucleotide exchange factor.	bind
3995	2	2268	5	10	NULL	0	NULL	Cdc24	GP		is					Cdc42 guanine nucleotide exchange factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_11_4116_s_211	16537494	( vii) Other authors  and our unpublished data show that the yeast epsins bind Cdc24, the Cdc42 guanine nucleotide exchange factor.	bind
3890	1	2268	6	10	NULL	0	NULL	epsins	GP	yeast	bind					Cdc24	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_11_4116_s_211	16537494	( vii) Other authors  and our unpublished data show that the yeast epsins bind Cdc24, the Cdc42 guanine nucleotide exchange factor.	bind
3891	2	2268	6	10	NULL	0	NULL	Cdc24	GP		is 					Cdc42 guanine nucleotide exchange factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_11_4116_s_211	16537494	( vii) Other authors  and our unpublished data show that the yeast epsins bind Cdc24, the Cdc42 guanine nucleotide exchange factor.	bind
3996	1	2270	5	10	NULL	0	NULL	Pax5 protein	GP	partially degraded	bind					CD19	GP			 site	NULL		NULL	NULL	NULL	NULL	gw70_genetics_171_3_1125_s_270	16079238	(*) indicates partially degraded Pax5  protein that still binds to the CD19 site.	bind
3892	1	2270	6	10	NULL	0	NULL	Pax5 protein	GP	partially degraded	bind					CD19	GP			site	NULL		NULL	NULL	NULL	NULL	gw70_genetics_171_3_1125_s_270	16079238	(*) indicates partially degraded Pax5  protein that still binds to the CD19 site.	bind
3997	1	2271	5	10	NULL	0	NULL	SREBP	GP		bind					LDLR	GP			SRE	NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_46_5_862_s_214	15716578	(+) Indicates the positive control reaction, in which SREBP is  bound with labeled LDL receptor (LDLR) SRE.	bind
3998	2	2271	5	10	NULL	0	NULL	LDLR	GP		is					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_46_5_862_s_214	15716578	(+) Indicates the positive control reaction, in which SREBP is  bound with labeled LDL receptor (LDLR) SRE.	bind
3893	1	2271	6	10	NULL	0	NULL	SREBP	GP		bind					LDL receptor	GP			SRE	NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_46_5_862_s_214	15716578	(+) Indicates the positive control reaction, in which SREBP is  bound with labeled LDL receptor (LDLR) SRE.	bind
4863	2	2271	6	10	NULL	0	NULL	LDLR	GP		is					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_46_5_862_s_214	15716578	(+) Indicates the positive control reaction, in which SREBP is  bound with labeled LDL receptor (LDLR) SRE.	bind
3999	1	2272	5	10	NULL	0	NULL	(+)-BPDE	Chemical		bind		covalently			guanine	Chemical				NULL	DNA	NULL	NULL	NULL	NULL	gw60_carcinogenesis_20_12_2279_s_13	10590220	(+)-BPDE covalently binds predominantly to guanine in DNA (10,11 and references therein) whereas ( - )-B[ c]PhDE binds preferentially to adenine in DNA ( 12, 13).	bind
4000	2	2272	5	10	NULL	0	NULL	( - )-BPhDE	Chemical		bind		preferentially			adenine	Chemical				NULL	DNA	NULL	NULL	NULL	NULL	gw60_carcinogenesis_20_12_2279_s_13	10590220	(+)-BPDE covalently binds predominantly to guanine in DNA (10,11 and references therein) whereas ( - )-B[ c]PhDE binds preferentially to adenine in DNA ( 12, 13).	bind
3894	1	2272	6	10	NULL	0	NULL	(+)-BPDE	Chemical		bind		covalently			guanine	Chemical				NULL	DNA	NULL	NULL	NULL	NULL	gw60_carcinogenesis_20_12_2279_s_13	10590220	(+)-BPDE covalently binds predominantly to guanine in DNA (10,11 and references therein) whereas ( - )-B[ c]PhDE binds preferentially to adenine in DNA ( 12, 13).	bind
3895	2	2272	6	10	NULL	0	NULL	( - )-BPhDE 	Chemical		bind		preferentially			adenine	Chemical				NULL	DNA	NULL	NULL	NULL	NULL	gw60_carcinogenesis_20_12_2279_s_13	10590220	(+)-BPDE covalently binds predominantly to guanine in DNA (10,11 and references therein) whereas ( - )-B[ c]PhDE binds preferentially to adenine in DNA ( 12, 13).	bind
4001	1	2273	5	10	NULL	0	NULL	MK-801	Chemical		non-competitive antagonist of					NMDA receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_423_3_376_s_3	9515743	(+)-MK-801 ((+)-5-methyl-10,11-dihydro-5 H-dibenzo[ a, d]cyclohepten-5,10-imine maleate) is a non-competitive  N-methyl- -aspartate (NMDA) receptor antagonist binding the phencyclidine (PCP) binding site of the receptors  [ 1.	bind
4002	2	2273	5	10	NULL	0	NULL	MK-801	Chemical		is					(+)-5-methyl-10,11-dihydro-5 H-dibenzo[ a, d]cyclohepten-5,10-imine maleate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_423_3_376_s_3	9515743	(+)-MK-801 ((+)-5-methyl-10,11-dihydro-5 H-dibenzo[ a, d]cyclohepten-5,10-imine maleate) is a non-competitive  N-methyl- -aspartate (NMDA) receptor antagonist binding the phencyclidine (PCP) binding site of the receptors  [ 1.	bind
4003	3	2273	5	10	NULL	0	NULL	NMDA	Chemical		is					N-methyl- -aspartate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_423_3_376_s_3	9515743	(+)-MK-801 ((+)-5-methyl-10,11-dihydro-5 H-dibenzo[ a, d]cyclohepten-5,10-imine maleate) is a non-competitive  N-methyl- -aspartate (NMDA) receptor antagonist binding the phencyclidine (PCP) binding site of the receptors  [ 1.	bind
4004	4	2273	5	10	NULL	0	NULL	statement 1	Process		bind					receptors	GP			PCP binding site	NULL		NULL	NULL	NULL	NULL	gw60_febslett_423_3_376_s_3	9515743	(+)-MK-801 ((+)-5-methyl-10,11-dihydro-5 H-dibenzo[ a, d]cyclohepten-5,10-imine maleate) is a non-competitive  N-methyl- -aspartate (NMDA) receptor antagonist binding the phencyclidine (PCP) binding site of the receptors  [ 1.	bind
4005	5	2273	5	10	NULL	0	NULL	PCP	Chemical		is					phencyclidine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_423_3_376_s_3	9515743	(+)-MK-801 ((+)-5-methyl-10,11-dihydro-5 H-dibenzo[ a, d]cyclohepten-5,10-imine maleate) is a non-competitive  N-methyl- -aspartate (NMDA) receptor antagonist binding the phencyclidine (PCP) binding site of the receptors  [ 1.	bind
3896	1	2273	6	10	NULL	0	NULL	(+)-5-methyl-10,11-dihydro-5 H-dibenzo cyclohepten-5,10-imine maleate	Chemical		non-competitive antagonist of 					NMDA receptor 	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_423_3_376_s_3	9515743	(+)-MK-801 ((+)-5-methyl-10,11-dihydro-5 H-dibenzo[ a, d]cyclohepten-5,10-imine maleate) is a non-competitive  N-methyl- -aspartate (NMDA) receptor antagonist binding the phencyclidine (PCP) binding site of the receptors  [ 1.	bind
3897	2	2273	6	10	NULL	0	NULL	NMDA	Chemical		is					N-methyl- -aspartate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_423_3_376_s_3	9515743	(+)-MK-801 ((+)-5-methyl-10,11-dihydro-5 H-dibenzo[ a, d]cyclohepten-5,10-imine maleate) is a non-competitive  N-methyl- -aspartate (NMDA) receptor antagonist binding the phencyclidine (PCP) binding site of the receptors  [ 1.	bind
3898	3	2273	6	10	NULL	0	NULL	statement 1	Process		bind					receptor 	GP			PCP binding site	NULL		NULL	NULL	NULL	NULL	gw60_febslett_423_3_376_s_3	9515743	(+)-MK-801 ((+)-5-methyl-10,11-dihydro-5 H-dibenzo[ a, d]cyclohepten-5,10-imine maleate) is a non-competitive  N-methyl- -aspartate (NMDA) receptor antagonist binding the phencyclidine (PCP) binding site of the receptors  [ 1.	bind
3899	4	2273	6	10	NULL	0	NULL	PCP	Chemical		is					phencyclidine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_423_3_376_s_3	9515743	(+)-MK-801 ((+)-5-methyl-10,11-dihydro-5 H-dibenzo[ a, d]cyclohepten-5,10-imine maleate) is a non-competitive  N-methyl- -aspartate (NMDA) receptor antagonist binding the phencyclidine (PCP) binding site of the receptors  [ 1.	bind
54263	5	2273	6	10	NULL	0	NULL	MK-801	Chemical		is					5-methyl-10,11-dihydro-5 H-dibenzo[ a, d]cyclohepten-5,10-imine maleate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_423_3_376_s_3	9515743	(+)-MK-801 ((+)-5-methyl-10,11-dihydro-5 H-dibenzo[ a, d]cyclohepten-5,10-imine maleate) is a non-competitive  N-methyl- -aspartate (NMDA) receptor antagonist binding the phencyclidine (PCP) binding site of the receptors  [ 1.	bind
4006	1	2274	5	10	NULL	0	NULL	amnesiac	GroupOfPeople		is deficient in					neuropeptide gene	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_20_3_445_s_421	9539121	(1)  amnesiac is deficient in a gene for a neuropeptide that binds to a G protein-coupled receptor that stimulates adenylyl cyclase (Feaney and Quinn, 1995).	bind
4007	2	2274	5	10	NULL	0	NULL	neuropeptide gene	GP		bind					G protein-coupled receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_20_3_445_s_421	9539121	(1)  amnesiac is deficient in a gene for a neuropeptide that binds to a G protein-coupled receptor that stimulates adenylyl cyclase (Feaney and Quinn, 1995).	bind
4008	3	2274	5	10	NULL	0	NULL	statement 2	Process		stimulate					adenylyl cyclase	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_20_3_445_s_421	9539121	(1)  amnesiac is deficient in a gene for a neuropeptide that binds to a G protein-coupled receptor that stimulates adenylyl cyclase (Feaney and Quinn, 1995).	bind
3900	1	2274	6	10	NULL	0	NULL	G protein-coupled receptor	GP		stimulates					adenylyl cyclase	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_20_3_445_s_421	9539121	(1)  amnesiac is deficient in a gene for a neuropeptide that binds to a G protein-coupled receptor that stimulates adenylyl cyclase (Feaney and Quinn, 1995).	bind
3901	2	2274	6	10	NULL	0	NULL	neuropeptide gene	GP		bind					G protein-coupled receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_20_3_445_s_421	9539121	(1)  amnesiac is deficient in a gene for a neuropeptide that binds to a G protein-coupled receptor that stimulates adenylyl cyclase (Feaney and Quinn, 1995).	bind
3902	3	2274	6	10	NULL	0	NULL	amnesiac	GroupOfPeople		is associated with					neuropeptide gene	GP	deficiency of			NULL		NULL	NULL	NULL	NULL	gw60_neuron_20_3_445_s_421	9539121	(1)  amnesiac is deficient in a gene for a neuropeptide that binds to a G protein-coupled receptor that stimulates adenylyl cyclase (Feaney and Quinn, 1995).	bind
4009	1	2275	5	10	NULL	0	NULL	PsbP	GP	chlamydomonas	bind		directly			PS II	GP	chlamydomonas			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_3	16049780	(1)  Chlamydomonas PsbP and PsbQ directly bound to Chlamydomonas PS II independent  of the other extrinsic proteins but not to spinach PS II.	bind
4010	2	2275	5	10	NULL	0	NULL	statement 1	Process		is independent of					extrinsic proteins	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_3	16049780	(1)  Chlamydomonas PsbP and PsbQ directly bound to Chlamydomonas PS II independent  of the other extrinsic proteins but not to spinach PS II.	bind
4011	3	2275	5	10	NULL	0	NULL	PsbQ	GP	chlamydomonas	bind		directly			PS II	GP	chlamydomonas			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_3	16049780	(1)  Chlamydomonas PsbP and PsbQ directly bound to Chlamydomonas PS II independent  of the other extrinsic proteins but not to spinach PS II.	bind
4012	4	2275	5	10	NULL	0	NULL	statement 3	Process		is independent of					extrinsic proteins	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_3	16049780	(1)  Chlamydomonas PsbP and PsbQ directly bound to Chlamydomonas PS II independent  of the other extrinsic proteins but not to spinach PS II.	bind
4013	5	2275	5	10	NULL	0	NULL	PsbP	GP	chlamydomonas	does not bind		directly			PS II	GP	spinach			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_3	16049780	(1)  Chlamydomonas PsbP and PsbQ directly bound to Chlamydomonas PS II independent  of the other extrinsic proteins but not to spinach PS II.	bind
4014	6	2275	5	10	NULL	0	NULL	PsbQ	GP	chlamydomonas	does not bind		directly			PS II	GP	spinach			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_3	16049780	(1)  Chlamydomonas PsbP and PsbQ directly bound to Chlamydomonas PS II independent  of the other extrinsic proteins but not to spinach PS II.	bind
3903	1	2275	6	10	NULL	0	NULL	PsbP	GP	Chlamydomonas	bind		directly			PSII	GP	Chlamydomonas			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_3	16049780	(1)  Chlamydomonas PsbP and PsbQ directly bound to Chlamydomonas PS II independent  of the other extrinsic proteins but not to spinach PS II.	bind
3904	2	2275	6	10	NULL	0	NULL	PsbQ	GP	Chlamydomonas	bind		directly			PS II	GP	Chlamydomonas			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_3	16049780	(1)  Chlamydomonas PsbP and PsbQ directly bound to Chlamydomonas PS II independent  of the other extrinsic proteins but not to spinach PS II.	bind
3905	3	2275	6	10	NULL	0	NULL	statement 1	Process		is independent of					extrinsic proteins	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_3	16049780	(1)  Chlamydomonas PsbP and PsbQ directly bound to Chlamydomonas PS II independent  of the other extrinsic proteins but not to spinach PS II.	bind
3906	4	2275	6	10	NULL	0	NULL	statement 2	GP		is independent of					extrinsic proteins	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_3	16049780	(1)  Chlamydomonas PsbP and PsbQ directly bound to Chlamydomonas PS II independent  of the other extrinsic proteins but not to spinach PS II.	bind
3907	5	2275	6	10	NULL	0	NULL	PsbP	GP	Chlamydomonas	does not bind					PS II	GP	spinach			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_3	16049780	(1)  Chlamydomonas PsbP and PsbQ directly bound to Chlamydomonas PS II independent  of the other extrinsic proteins but not to spinach PS II.	bind
3908	6	2275	6	10	NULL	0	NULL	PsbQ	GP	Chlamydomonas	does not bind					PS II	GP	spinach			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_3	16049780	(1)  Chlamydomonas PsbP and PsbQ directly bound to Chlamydomonas PS II independent  of the other extrinsic proteins but not to spinach PS II.	bind
4015	1	2276	5	10	NULL	0	NULL	US11	GP		bind			lumenal domain		MHCI 	GP		heavy chain substrate		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_9_3690_s_222	12972557	(1) After insertion into the ER, the lumenal  domain of US11 binds to the MHCI heavy chain substrate, possibly in a complex with  beta2m (recognition).	bind
4016	2	2276	5	10	NULL	0	NULL	statement 1	Process		is in complex with		possibly			 beta2m	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_9_3690_s_222	12972557	(1) After insertion into the ER, the lumenal  domain of US11 binds to the MHCI heavy chain substrate, possibly in a complex with  beta2m (recognition).	bind
4017	4	2276	5	10	NULL	0	NULL	statement 1	Process		occurs after					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_9_3690_s_222	12972557	(1) After insertion into the ER, the lumenal  domain of US11 binds to the MHCI heavy chain substrate, possibly in a complex with  beta2m (recognition).	bind
5247	3	2276	5	10	NULL	0	NULL				insert into			Lumenal domain		ER	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_9_3690_s_222	12972557	(1) After insertion into the ER, the lumenal  domain of US11 binds to the MHCI heavy chain substrate, possibly in a complex with  beta2m (recognition).	bind
3909	1	2276	6	10	NULL	0	NULL	US11	NULL		bind	NULL		lumenal domain		MHCI	NULL		heavy chain substrate		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_9_3690_s_222	12972557	(1) After insertion into the ER, the lumenal  domain of US11 binds to the MHCI heavy chain substrate, possibly in a complex with  beta2m (recognition).	bind
3910	2	2276	6	10	NULL	0	NULL	US11	GP		forms complex with		possibly			beta2m	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_9_3690_s_222	12972557	(1) After insertion into the ER, the lumenal  domain of US11 binds to the MHCI heavy chain substrate, possibly in a complex with  beta2m (recognition).	bind
4864	3	2276	6	10	NULL	0	NULL				insert into			lumenal domain		ER	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_9_3690_s_222	12972557	(1) After insertion into the ER, the lumenal  domain of US11 binds to the MHCI heavy chain substrate, possibly in a complex with  beta2m (recognition).	bind
4865	4	2276	6	10	NULL	0	NULL	statement 1	Process		occurs after					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_9_3690_s_222	12972557	(1) After insertion into the ER, the lumenal  domain of US11 binds to the MHCI heavy chain substrate, possibly in a complex with  beta2m (recognition).	bind
4018	1	2277	5	10	NULL	0	NULL	Nef	GP		bind			acidic cluster 62EEEE65		PACS-1/AP-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_111_6_853_s_286	12526811	(1) Binding of Nef acidic cluster 62EEEE65 to PACS-1/AP-1 targets Nef to the TGN.	bind
4019	2	2277	5	10	NULL	0	NULL	Nef	GP		is targeted to					TGN	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cell_111_6_853_s_286	12526811	(1) Binding of Nef acidic cluster 62EEEE65 to PACS-1/AP-1 targets Nef to the TGN.	bind
4020	3	2277	5	10	NULL	0	NULL	statement 1	Process		is necessary for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_111_6_853_s_286	12526811	(1) Binding of Nef acidic cluster 62EEEE65 to PACS-1/AP-1 targets Nef to the TGN.	bind
3911	1	2277	6	10	NULL	0	NULL	Nef	GP		bind			acidic cluster 62EEEE65		PACS-1/AP-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_111_6_853_s_286	12526811	(1) Binding of Nef acidic cluster 62EEEE65 to PACS-1/AP-1 targets Nef to the TGN.	bind
3913	2	2277	6	10	NULL	0	NULL	Nef	GP		targeted to					TGN	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cell_111_6_853_s_286	12526811	(1) Binding of Nef acidic cluster 62EEEE65 to PACS-1/AP-1 targets Nef to the TGN.	bind
3914	3	2277	6	10	NULL	0	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_111_6_853_s_286	12526811	(1) Binding of Nef acidic cluster 62EEEE65 to PACS-1/AP-1 targets Nef to the TGN.	bind
4021	1	2278	5	10	NULL	0	NULL	Cdc42	GP		bind								GBD		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_13_7_534_s_215	12676083	(1) Cdc42 binding to the GBD disrupts the autoregulatory interaction with DAD  [13]  , and (2) the GTPase-Drf3 complex becomes recruited to the cell cortex.	bind
4022	2	2278	5	10	NULL	0	NULL	statement 1	Process		disrupt							autoregulatory interaction with	DAD		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_13_7_534_s_215	12676083	(1) Cdc42 binding to the GBD disrupts the autoregulatory interaction with DAD  [13]  , and (2) the GTPase-Drf3 complex becomes recruited to the cell cortex.	bind
4023	3	2278	5	10	NULL	0	NULL	GTPase-Drf3 complex	GP		is recruited to					cell cortex	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_13_7_534_s_215	12676083	(1) Cdc42 binding to the GBD disrupts the autoregulatory interaction with DAD  [13]  , and (2) the GTPase-Drf3 complex becomes recruited to the cell cortex.	bind
46422	4	2278	5	10	NULL	0	NULL	statement 1	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_13_7_534_s_215	12676083	(1) Cdc42 binding to the GBD disrupts the autoregulatory interaction with DAD  [13]  , and (2) the GTPase-Drf3 complex becomes recruited to the cell cortex.	bind
3916	1	2278	6	10	NULL	0	NULL	Cdc42	GP		bind								GBD		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_13_7_534_s_215	12676083	(1) Cdc42 binding to the GBD disrupts the autoregulatory interaction with DAD  [13]  , and (2) the GTPase-Drf3 complex becomes recruited to the cell cortex.	bind
3917	2	2278	6	10	NULL	0	NULL	statement 1	Process		disrupts							autoregulatory interaction with	DAD		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_13_7_534_s_215	12676083	(1) Cdc42 binding to the GBD disrupts the autoregulatory interaction with DAD  [13]  , and (2) the GTPase-Drf3 complex becomes recruited to the cell cortex.	bind
3918	3	2278	6	10	NULL	0	NULL	GTPase-Drf3 complex	GP	complex	is recruited					cell cortex	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_13_7_534_s_215	12676083	(1) Cdc42 binding to the GBD disrupts the autoregulatory interaction with DAD  [13]  , and (2) the GTPase-Drf3 complex becomes recruited to the cell cortex.	bind
3919	4	2278	6	10	NULL	0	NULL	statement 1	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_13_7_534_s_215	12676083	(1) Cdc42 binding to the GBD disrupts the autoregulatory interaction with DAD  [13]  , and (2) the GTPase-Drf3 complex becomes recruited to the cell cortex.	bind
4269	1	2279	5	10	NULL	0	NULL	cholera toxin	GP		bind		selectively	B subunit		excitatory opioid receptors	GP	putative;; allosteric	GM1 regulatory site		NULL	mice	NULL	NULL	NULL	NULL	gw60_brainres_888_1_75_s_132	11146054	(1) Cotreatment of mice with low doses of cholera toxin-B subunit (ca. 10  g/kg, i.p.), which binds selectively to a putative allosteric GM1 regulatory site on excitatory opioid receptors [ 12,   30,  31 and   37], blocks opioid-induced hyperalgesia and unmasks potent opioid analgesia (Shen and Crain, in preparation), comparable to the effects of ultra-low-dose NTX.	bind
4270	2	2279	5	10	NULL	0	NULL	opioid	Chemical		induce					hyperalgesia	MedicalFinding				NULL	mice	NULL	NULL	NULL	NULL	gw60_brainres_888_1_75_s_132	11146054	(1) Cotreatment of mice with low doses of cholera toxin-B subunit (ca. 10  g/kg, i.p.), which binds selectively to a putative allosteric GM1 regulatory site on excitatory opioid receptors [ 12,   30,  31 and   37], blocks opioid-induced hyperalgesia and unmasks potent opioid analgesia (Shen and Crain, in preparation), comparable to the effects of ultra-low-dose NTX.	bind
4271	3	2279	5	10	NULL	0	NULL	statement 1	Process		blocks					statement 2	Process				NULL	mice	NULL	NULL	NULL	NULL	gw60_brainres_888_1_75_s_132	11146054	(1) Cotreatment of mice with low doses of cholera toxin-B subunit (ca. 10  g/kg, i.p.), which binds selectively to a putative allosteric GM1 regulatory site on excitatory opioid receptors [ 12,   30,  31 and   37], blocks opioid-induced hyperalgesia and unmasks potent opioid analgesia (Shen and Crain, in preparation), comparable to the effects of ultra-low-dose NTX.	bind
46423	4	2279	5	10	NULL	0	NULL	statement 1	Process		unmasks					opioid analgesia	MedicalFinding	potent			NULL	mice	NULL	NULL	NULL	NULL	gw60_brainres_888_1_75_s_132	11146054	(1) Cotreatment of mice with low doses of cholera toxin-B subunit (ca. 10  g/kg, i.p.), which binds selectively to a putative allosteric GM1 regulatory site on excitatory opioid receptors [ 12,   30,  31 and   37], blocks opioid-induced hyperalgesia and unmasks potent opioid analgesia (Shen and Crain, in preparation), comparable to the effects of ultra-low-dose NTX.	bind
3920	1	2279	6	10	NULL	0	NULL	cholera toxin	GP		bind		selectively	B subunit		excitatory opioid receptors	GP	putative;; allosteric	GM1 regulatory site		NULL	mice	NULL	NULL	NULL	NULL	gw60_brainres_888_1_75_s_132	11146054	(1) Cotreatment of mice with low doses of cholera toxin-B subunit (ca. 10  g/kg, i.p.), which binds selectively to a putative allosteric GM1 regulatory site on excitatory opioid receptors [ 12,   30,  31 and   37], blocks opioid-induced hyperalgesia and unmasks potent opioid analgesia (Shen and Crain, in preparation), comparable to the effects of ultra-low-dose NTX.	bind
3921	3	2279	6	10	NULL	0	NULL	statement 1	Process		blocks					statement 2	Process				NULL	mice	NULL	NULL	NULL	NULL	gw60_brainres_888_1_75_s_132	11146054	(1) Cotreatment of mice with low doses of cholera toxin-B subunit (ca. 10  g/kg, i.p.), which binds selectively to a putative allosteric GM1 regulatory site on excitatory opioid receptors [ 12,   30,  31 and   37], blocks opioid-induced hyperalgesia and unmasks potent opioid analgesia (Shen and Crain, in preparation), comparable to the effects of ultra-low-dose NTX.	bind
3922	4	2279	6	10	NULL	0	NULL	statement 1	Process		unmasks					opioid analgesia	MedicalFinding	potent			NULL	mice	NULL	NULL	NULL	NULL	gw60_brainres_888_1_75_s_132	11146054	(1) Cotreatment of mice with low doses of cholera toxin-B subunit (ca. 10  g/kg, i.p.), which binds selectively to a putative allosteric GM1 regulatory site on excitatory opioid receptors [ 12,   30,  31 and   37], blocks opioid-induced hyperalgesia and unmasks potent opioid analgesia (Shen and Crain, in preparation), comparable to the effects of ultra-low-dose NTX.	bind
46424	2	2279	6	10	NULL	0	NULL	opiod	Chemical		induce					hyperalgesia	MedicalFinding				NULL	mice	NULL	NULL	NULL	NULL	gw60_brainres_888_1_75_s_132	11146054	(1) Cotreatment of mice with low doses of cholera toxin-B subunit (ca. 10  g/kg, i.p.), which binds selectively to a putative allosteric GM1 regulatory site on excitatory opioid receptors [ 12,   30,  31 and   37], blocks opioid-induced hyperalgesia and unmasks potent opioid analgesia (Shen and Crain, in preparation), comparable to the effects of ultra-low-dose NTX.	bind
4024	1	2280	5	10	NULL	0	NULL	Cyclin D	GP		bind					Cdk4	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_8_2703_s_120	10436023	(1) Cyclin D binds Cdk4; the filled circle (node) on the line represents the CycD:Cdk4 complex itself.	bind
46425	2	2280	5	10	NULL	0	NULL	statement 1	Process		forms					CycD:Cdk4 complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_8_2703_s_120	10436023	(1) Cyclin D binds Cdk4; the filled circle (node) on the line represents the CycD:Cdk4 complex itself.	bind
3923	1	2280	6	10	NULL	0	NULL	Cyclin D	GP		bind					Cdk4	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_8_2703_s_120	10436023	(1) Cyclin D binds Cdk4; the filled circle (node) on the line represents the CycD:Cdk4 complex itself.	bind
3924	2	2280	6	10	NULL	0	NULL	statement 1	Process		forms 					CycD:Cdk4 complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_8_2703_s_120	10436023	(1) Cyclin D binds Cdk4; the filled circle (node) on the line represents the CycD:Cdk4 complex itself.	bind
4039	1	2281	5	10	NULL	0	NULL	cortisol	Chemical		bind					Type I (mineralocorticoid) receptor	GP	human			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_kidney-int_42_6_1474763_s_2	1474763	(1) Decreased 11 beta-OHSD activity permits binding of cortisol to the  Type I (mineralocorticoid) receptor in humans, thereby producing spironolactone-inhibitable  Na+ retention, hypokalemia and hypertension, the syndrome of apparent mineralocorticoid  excess (AME).	bind
4040	2	2281	5	10	NULL	0	NULL	11 beta-OHSD	GP	decreased activity	permit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_kidney-int_42_6_1474763_s_2	1474763	(1) Decreased 11 beta-OHSD activity permits binding of cortisol to the  Type I (mineralocorticoid) receptor in humans, thereby producing spironolactone-inhibitable  Na+ retention, hypokalemia and hypertension, the syndrome of apparent mineralocorticoid  excess (AME).	bind
4042	3	2281	5	10	NULL	0	NULL	AME	MedicalFinding		is					 apparent mineralocorticoid excess	MedicalFinding				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_kidney-int_42_6_1474763_s_2	1474763	(1) Decreased 11 beta-OHSD activity permits binding of cortisol to the  Type I (mineralocorticoid) receptor in humans, thereby producing spironolactone-inhibitable  Na+ retention, hypokalemia and hypertension, the syndrome of apparent mineralocorticoid  excess (AME).	bind
5248	8	2281	5	10	NULL	0	NULL	AME	MedicalFinding		is associated with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_kidney-int_42_6_1474763_s_2	1474763	(1) Decreased 11 beta-OHSD activity permits binding of cortisol to the  Type I (mineralocorticoid) receptor in humans, thereby producing spironolactone-inhibitable  Na+ retention, hypokalemia and hypertension, the syndrome of apparent mineralocorticoid  excess (AME).	bind
5249	9	2281	5	10	NULL	0	NULL	AME	MedicalFinding		is associated with					statement 5	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_kidney-int_42_6_1474763_s_2	1474763	(1) Decreased 11 beta-OHSD activity permits binding of cortisol to the  Type I (mineralocorticoid) receptor in humans, thereby producing spironolactone-inhibitable  Na+ retention, hypokalemia and hypertension, the syndrome of apparent mineralocorticoid  excess (AME).	bind
5250	10	2281	5	10	NULL	0	NULL	AME	MedicalFinding		is associated with					statement 6	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_kidney-int_42_6_1474763_s_2	1474763	(1) Decreased 11 beta-OHSD activity permits binding of cortisol to the  Type I (mineralocorticoid) receptor in humans, thereby producing spironolactone-inhibitable  Na+ retention, hypokalemia and hypertension, the syndrome of apparent mineralocorticoid  excess (AME).	bind
46692	4	2281	5	10	NULL	0	NULL	Na+ retention	Process		is inhibited by					spironolactone	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_kidney-int_42_6_1474763_s_2	1474763	(1) Decreased 11 beta-OHSD activity permits binding of cortisol to the  Type I (mineralocorticoid) receptor in humans, thereby producing spironolactone-inhibitable  Na+ retention, hypokalemia and hypertension, the syndrome of apparent mineralocorticoid  excess (AME).	bind
46693	5	2281	5	10	NULL	0	NULL	statement 2	Process		produce					statement 4	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_kidney-int_42_6_1474763_s_2	1474763	(1) Decreased 11 beta-OHSD activity permits binding of cortisol to the  Type I (mineralocorticoid) receptor in humans, thereby producing spironolactone-inhibitable  Na+ retention, hypokalemia and hypertension, the syndrome of apparent mineralocorticoid  excess (AME).	bind
46694	6	2281	5	10	NULL	0	NULL	statement 2	Process		produce					hypokalemia	MedicalFinding				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_kidney-int_42_6_1474763_s_2	1474763	(1) Decreased 11 beta-OHSD activity permits binding of cortisol to the  Type I (mineralocorticoid) receptor in humans, thereby producing spironolactone-inhibitable  Na+ retention, hypokalemia and hypertension, the syndrome of apparent mineralocorticoid  excess (AME).	bind
46695	7	2281	5	10	NULL	0	NULL	statement 2	Process		produce					hypertension	MedicalFinding				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_kidney-int_42_6_1474763_s_2	1474763	(1) Decreased 11 beta-OHSD activity permits binding of cortisol to the  Type I (mineralocorticoid) receptor in humans, thereby producing spironolactone-inhibitable  Na+ retention, hypokalemia and hypertension, the syndrome of apparent mineralocorticoid  excess (AME).	bind
3955	1	2281	6	10	NULL	0	NULL	cortisol	Chemical		bind					Type I mineralocorticoid receptor	GP	human			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_kidney-int_42_6_1474763_s_2	1474763	(1) Decreased 11 beta-OHSD activity permits binding of cortisol to the  Type I (mineralocorticoid) receptor in humans, thereby producing spironolactone-inhibitable  Na+ retention, hypokalemia and hypertension, the syndrome of apparent mineralocorticoid  excess (AME).	bind
3956	2	2281	6	10	NULL	0	NULL	11 beta-OHSD 	GP	decreased activity of	permits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_kidney-int_42_6_1474763_s_2	1474763	(1) Decreased 11 beta-OHSD activity permits binding of cortisol to the  Type I (mineralocorticoid) receptor in humans, thereby producing spironolactone-inhibitable  Na+ retention, hypokalemia and hypertension, the syndrome of apparent mineralocorticoid  excess (AME).	bind
3957	3	2281	6	10	NULL	0	NULL	Na+ retention	Process		is inhibited by					spironolactone	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_kidney-int_42_6_1474763_s_2	1474763	(1) Decreased 11 beta-OHSD activity permits binding of cortisol to the  Type I (mineralocorticoid) receptor in humans, thereby producing spironolactone-inhibitable  Na+ retention, hypokalemia and hypertension, the syndrome of apparent mineralocorticoid  excess (AME).	bind
3958	4	2281	6	10	NULL	0	NULL	statement 2	Process		produce					statement 3	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_kidney-int_42_6_1474763_s_2	1474763	(1) Decreased 11 beta-OHSD activity permits binding of cortisol to the  Type I (mineralocorticoid) receptor in humans, thereby producing spironolactone-inhibitable  Na+ retention, hypokalemia and hypertension, the syndrome of apparent mineralocorticoid  excess (AME).	bind
3959	5	2281	6	10	NULL	0	NULL	statement 2	Process		produce					hypokalemia	MedicalFinding				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_kidney-int_42_6_1474763_s_2	1474763	(1) Decreased 11 beta-OHSD activity permits binding of cortisol to the  Type I (mineralocorticoid) receptor in humans, thereby producing spironolactone-inhibitable  Na+ retention, hypokalemia and hypertension, the syndrome of apparent mineralocorticoid  excess (AME).	bind
4603	7	2281	6	10	NULL	0	NULL	AME	MedicalFinding		is					apparent mineralocorticoid excess	MedicalFinding				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_kidney-int_42_6_1474763_s_2	1474763	(1) Decreased 11 beta-OHSD activity permits binding of cortisol to the  Type I (mineralocorticoid) receptor in humans, thereby producing spironolactone-inhibitable  Na+ retention, hypokalemia and hypertension, the syndrome of apparent mineralocorticoid  excess (AME).	bind
4605	8	2281	6	10	NULL	0	NULL	AME	MedicalFinding		is associated with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_kidney-int_42_6_1474763_s_2	1474763	(1) Decreased 11 beta-OHSD activity permits binding of cortisol to the  Type I (mineralocorticoid) receptor in humans, thereby producing spironolactone-inhibitable  Na+ retention, hypokalemia and hypertension, the syndrome of apparent mineralocorticoid  excess (AME).	bind
4606	10	2281	6	10	NULL	0	NULL	AME	MedicalFinding		is associated with					statement 6	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_kidney-int_42_6_1474763_s_2	1474763	(1) Decreased 11 beta-OHSD activity permits binding of cortisol to the  Type I (mineralocorticoid) receptor in humans, thereby producing spironolactone-inhibitable  Na+ retention, hypokalemia and hypertension, the syndrome of apparent mineralocorticoid  excess (AME).	bind
4610	9	2281	6	10	NULL	0	NULL	AME	MedicalFinding		is associated with					statement 5	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_kidney-int_42_6_1474763_s_2	1474763	(1) Decreased 11 beta-OHSD activity permits binding of cortisol to the  Type I (mineralocorticoid) receptor in humans, thereby producing spironolactone-inhibitable  Na+ retention, hypokalemia and hypertension, the syndrome of apparent mineralocorticoid  excess (AME).	bind
46696	6	2281	6	10	NULL	0	NULL	statement 2	Process		produce					hypertension	MedicalFinding				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_kidney-int_42_6_1474763_s_2	1474763	(1) Decreased 11 beta-OHSD activity permits binding of cortisol to the  Type I (mineralocorticoid) receptor in humans, thereby producing spironolactone-inhibitable  Na+ retention, hypokalemia and hypertension, the syndrome of apparent mineralocorticoid  excess (AME).	bind
4043	1	2282	5	10	NULL	0	NULL	Arp2/3	GP		bind					F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jneurosci_26_5_1579_s_145	16452681	(1) Ena/VASP inhibits Arp2/3 binding to F-actin, thereby decreasing F-actin branching and lamellipodia formation (Krause et al., 2003 ).	bind
4044	2	2282	5	10	NULL	0	NULL	Ena/VASP	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jneurosci_26_5_1579_s_145	16452681	(1) Ena/VASP inhibits Arp2/3 binding to F-actin, thereby decreasing F-actin branching and lamellipodia formation (Krause et al., 2003 ).	bind
4045	3	2282	5	10	NULL	0	NULL	statement 2	Process		decrease					F-actin	GP	branching of			NULL		NULL	NULL	NULL	NULL	gw70_jneurosci_26_5_1579_s_145	16452681	(1) Ena/VASP inhibits Arp2/3 binding to F-actin, thereby decreasing F-actin branching and lamellipodia formation (Krause et al., 2003 ).	bind
4046	4	2282	5	10	NULL	0	NULL	statement 2	Process		decrease					lamellipodia	CellComponent	formation of			NULL		NULL	NULL	NULL	NULL	gw70_jneurosci_26_5_1579_s_145	16452681	(1) Ena/VASP inhibits Arp2/3 binding to F-actin, thereby decreasing F-actin branching and lamellipodia formation (Krause et al., 2003 ).	bind
3961	1	2282	6	10	NULL	0	NULL	Arp2/3	GP		bind					F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jneurosci_26_5_1579_s_145	16452681	(1) Ena/VASP inhibits Arp2/3 binding to F-actin, thereby decreasing F-actin branching and lamellipodia formation (Krause et al., 2003 ).	bind
3962	2	2282	6	10	NULL	0	NULL	Ena/VASP	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jneurosci_26_5_1579_s_145	16452681	(1) Ena/VASP inhibits Arp2/3 binding to F-actin, thereby decreasing F-actin branching and lamellipodia formation (Krause et al., 2003 ).	bind
3963	3	2282	6	10	NULL	0	NULL	statement 2	Process		decreases					F-actin	GP	branching of 			NULL		NULL	NULL	NULL	NULL	gw70_jneurosci_26_5_1579_s_145	16452681	(1) Ena/VASP inhibits Arp2/3 binding to F-actin, thereby decreasing F-actin branching and lamellipodia formation (Krause et al., 2003 ).	bind
3964	4	2282	6	10	NULL	0	NULL	statement 2	Process		decreases					lamellipodia 	CellComponent	formation of			NULL		NULL	NULL	NULL	NULL	gw70_jneurosci_26_5_1579_s_145	16452681	(1) Ena/VASP inhibits Arp2/3 binding to F-actin, thereby decreasing F-actin branching and lamellipodia formation (Krause et al., 2003 ).	bind
4047	1	2283	5	10	NULL	0	NULL	THDOC	Chemical		inhibit					TBPS	Chemical	 binding of			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_21_1_330_s_225	11150350	(1) It decreased the fraction of [35]TBPS binding inhibited by THDOC (Fig.  1), suggesting a decrease in sensitivity to THDOC, and (2) it enhanced the potentiation of [35]TBPS binding by GABA in stratum oriens and attenuated the inhibition of [35]TBPS binding by GABA in stratum radiatum (Fig.  3).	bind
4048	2	2283	5	10	NULL	0	NULL	statement 1	Process		decrease					THDOC	Chemical	sensitivity to			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_21_1_330_s_225	11150350	(1) It decreased the fraction of [35]TBPS binding inhibited by THDOC (Fig.  1), suggesting a decrease in sensitivity to THDOC, and (2) it enhanced the potentiation of [35]TBPS binding by GABA in stratum oriens and attenuated the inhibition of [35]TBPS binding by GABA in stratum radiatum (Fig.  3).	bind
5256	3	2283	5	10	NULL	0	NULL	GABA	Chemical		bind					TBPS	Chemical				NULL	stratium oriens	NULL	NULL	NULL	NULL	gw60_jneurosci_21_1_330_s_225	11150350	(1) It decreased the fraction of [35]TBPS binding inhibited by THDOC (Fig.  1), suggesting a decrease in sensitivity to THDOC, and (2) it enhanced the potentiation of [35]TBPS binding by GABA in stratum oriens and attenuated the inhibition of [35]TBPS binding by GABA in stratum radiatum (Fig.  3).	bind
5257	4	2283	5	10	NULL	0	NULL	GABA	Chemical		bind					TBPS	Chemical				NULL	stratum radiatum	NULL	NULL	NULL	NULL	gw60_jneurosci_21_1_330_s_225	11150350	(1) It decreased the fraction of [35]TBPS binding inhibited by THDOC (Fig.  1), suggesting a decrease in sensitivity to THDOC, and (2) it enhanced the potentiation of [35]TBPS binding by GABA in stratum oriens and attenuated the inhibition of [35]TBPS binding by GABA in stratum radiatum (Fig.  3).	bind
4612	1	2283	6	10	NULL	0	NULL	THDOC	Chemical		inhibits					TBPS	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_21_1_330_s_225	11150350	(1) It decreased the fraction of [35]TBPS binding inhibited by THDOC (Fig.  1), suggesting a decrease in sensitivity to THDOC, and (2) it enhanced the potentiation of [35]TBPS binding by GABA in stratum oriens and attenuated the inhibition of [35]TBPS binding by GABA in stratum radiatum (Fig.  3).	bind
4613	2	2283	6	10	NULL	0	NULL	GABA	Chemical		bind					TBPS	Chemical				NULL	stratum oriens	NULL	NULL	NULL	NULL	gw60_jneurosci_21_1_330_s_225	11150350	(1) It decreased the fraction of [35]TBPS binding inhibited by THDOC (Fig.  1), suggesting a decrease in sensitivity to THDOC, and (2) it enhanced the potentiation of [35]TBPS binding by GABA in stratum oriens and attenuated the inhibition of [35]TBPS binding by GABA in stratum radiatum (Fig.  3).	bind
4614	3	2283	6	10	NULL	0	NULL	GABA	Chemical		bind					TBPS	Chemical				NULL	stratum radiatum	NULL	NULL	NULL	NULL	gw60_jneurosci_21_1_330_s_225	11150350	(1) It decreased the fraction of [35]TBPS binding inhibited by THDOC (Fig.  1), suggesting a decrease in sensitivity to THDOC, and (2) it enhanced the potentiation of [35]TBPS binding by GABA in stratum oriens and attenuated the inhibition of [35]TBPS binding by GABA in stratum radiatum (Fig.  3).	bind
4866	4	2283	6	10	NULL	0	NULL	statement 1	Process		decrease					THDOC	Chemical	sensitivity to			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_21_1_330_s_225	11150350	(1) It decreased the fraction of [35]TBPS binding inhibited by THDOC (Fig.  1), suggesting a decrease in sensitivity to THDOC, and (2) it enhanced the potentiation of [35]TBPS binding by GABA in stratum oriens and attenuated the inhibition of [35]TBPS binding by GABA in stratum radiatum (Fig.  3).	bind
4050	1	2284	5	10	NULL	0	NULL	CbbR	GP		does not bind									cbbR-cbbL intergenic region	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_4_1245_s_235	12562794	(1) No CbbR bound to the  cbbR-cbbL intergenic region.	bind
3965	1	2284	6	10	NULL	0	NULL	CbbR	GP		does not bind									cbbR-cbbL intergenic region	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_4_1245_s_235	12562794	(1) No CbbR bound to the  cbbR-cbbL intergenic region.	bind
4106	1	2285	5	10	NULL	0	NULL	CGS 21680	Chemical		bind		poorly			A1 receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_112_2_319_s_171	12044450	(1) Numerous studies have shown that CGS 21680 binds poorly to A1 receptors with a  Ki close to 1  M.	bind
3966	1	2285	6	10	NULL	0	NULL	CGS 21680	Chemical		bind		poorly			A1 receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_112_2_319_s_171	12044450	(1) Numerous studies have shown that CGS 21680 binds poorly to A1 receptors with a  Ki close to 1  M.	bind
4107	1	2286	5	10	NULL	0	NULL	nucleotide	NucleicAcid		bind								cleft 1		NULL		NULL	NULL	NULL	NULL	gw70_nature_422_6929_330_s_139	12646924	(1) The adenylation reaction involves nucleotide binding  to cleft 1 and NEDD8 binding to cleft 2; (2) the catalytic cysteine, facing NEDD8,  forms a thioester with NEDD8; (3) a second molecule of NEDD8 is adenylated; (4) occupation  of the nucleotide-binding pocket facilitates binding of E2 in cleft 1, promoting  transfer of the E1 thioester-linked Ublp to E2.	bind
4108	2	2286	5	10	NULL	0	NULL	NEDD8	GP		bind								cleft 2		NULL		NULL	NULL	NULL	NULL	gw70_nature_422_6929_330_s_139	12646924	(1) The adenylation reaction involves nucleotide binding  to cleft 1 and NEDD8 binding to cleft 2; (2) the catalytic cysteine, facing NEDD8,  forms a thioester with NEDD8; (3) a second molecule of NEDD8 is adenylated; (4) occupation  of the nucleotide-binding pocket facilitates binding of E2 in cleft 1, promoting  transfer of the E1 thioester-linked Ublp to E2.	bind
4109	3	2286	5	10	NULL	0	NULL	adenylation reaction	Process		involves					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_nature_422_6929_330_s_139	12646924	(1) The adenylation reaction involves nucleotide binding  to cleft 1 and NEDD8 binding to cleft 2; (2) the catalytic cysteine, facing NEDD8,  forms a thioester with NEDD8; (3) a second molecule of NEDD8 is adenylated; (4) occupation  of the nucleotide-binding pocket facilitates binding of E2 in cleft 1, promoting  transfer of the E1 thioester-linked Ublp to E2.	bind
4110	4	2286	5	10	NULL	0	NULL	adenylation reaction	Process		involves					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_nature_422_6929_330_s_139	12646924	(1) The adenylation reaction involves nucleotide binding  to cleft 1 and NEDD8 binding to cleft 2; (2) the catalytic cysteine, facing NEDD8,  forms a thioester with NEDD8; (3) a second molecule of NEDD8 is adenylated; (4) occupation  of the nucleotide-binding pocket facilitates binding of E2 in cleft 1, promoting  transfer of the E1 thioester-linked Ublp to E2.	bind
4112	5	2286	5	10	NULL	0	NULL	cysteine	AminoAcid	catalytic	forms					NEDD8	GP	thioester with			NULL		NULL	NULL	NULL	NULL	gw70_nature_422_6929_330_s_139	12646924	(1) The adenylation reaction involves nucleotide binding  to cleft 1 and NEDD8 binding to cleft 2; (2) the catalytic cysteine, facing NEDD8,  forms a thioester with NEDD8; (3) a second molecule of NEDD8 is adenylated; (4) occupation  of the nucleotide-binding pocket facilitates binding of E2 in cleft 1, promoting  transfer of the E1 thioester-linked Ublp to E2.	bind
4113	6	2286	5	10	NULL	0	NULL	NEDD8	GP		undergoes					adenylation	Process				NULL		NULL	NULL	NULL	NULL	gw70_nature_422_6929_330_s_139	12646924	(1) The adenylation reaction involves nucleotide binding  to cleft 1 and NEDD8 binding to cleft 2; (2) the catalytic cysteine, facing NEDD8,  forms a thioester with NEDD8; (3) a second molecule of NEDD8 is adenylated; (4) occupation  of the nucleotide-binding pocket facilitates binding of E2 in cleft 1, promoting  transfer of the E1 thioester-linked Ublp to E2.	bind
4114	7	2286	5	10	NULL	0	NULL	E2	GP		bind								cleft 1		NULL		NULL	NULL	NULL	NULL	gw70_nature_422_6929_330_s_139	12646924	(1) The adenylation reaction involves nucleotide binding  to cleft 1 and NEDD8 binding to cleft 2; (2) the catalytic cysteine, facing NEDD8,  forms a thioester with NEDD8; (3) a second molecule of NEDD8 is adenylated; (4) occupation  of the nucleotide-binding pocket facilitates binding of E2 in cleft 1, promoting  transfer of the E1 thioester-linked Ublp to E2.	bind
4115	8	2286	5	10	NULL	0	NULL	nucleotide-binding pocket	NucleicAcid	occupation of	facilitate					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw70_nature_422_6929_330_s_139	12646924	(1) The adenylation reaction involves nucleotide binding  to cleft 1 and NEDD8 binding to cleft 2; (2) the catalytic cysteine, facing NEDD8,  forms a thioester with NEDD8; (3) a second molecule of NEDD8 is adenylated; (4) occupation  of the nucleotide-binding pocket facilitates binding of E2 in cleft 1, promoting  transfer of the E1 thioester-linked Ublp to E2.	bind
4116	9	2286	5	10	NULL	0	NULL	Ublp	GP	E1 thioester-linked	is transferred to					E2	GP				NULL		NULL	NULL	NULL	NULL	gw70_nature_422_6929_330_s_139	12646924	(1) The adenylation reaction involves nucleotide binding  to cleft 1 and NEDD8 binding to cleft 2; (2) the catalytic cysteine, facing NEDD8,  forms a thioester with NEDD8; (3) a second molecule of NEDD8 is adenylated; (4) occupation  of the nucleotide-binding pocket facilitates binding of E2 in cleft 1, promoting  transfer of the E1 thioester-linked Ublp to E2.	bind
4117	10	2286	5	10	NULL	0	NULL	statement 8	Process		promote					statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw70_nature_422_6929_330_s_139	12646924	(1) The adenylation reaction involves nucleotide binding  to cleft 1 and NEDD8 binding to cleft 2; (2) the catalytic cysteine, facing NEDD8,  forms a thioester with NEDD8; (3) a second molecule of NEDD8 is adenylated; (4) occupation  of the nucleotide-binding pocket facilitates binding of E2 in cleft 1, promoting  transfer of the E1 thioester-linked Ublp to E2.	bind
3967	1	2286	6	10	NULL	0	NULL	nucleotide	NucleicAcid		bind								cleft 1		NULL		NULL	NULL	NULL	NULL	gw70_nature_422_6929_330_s_139	12646924	(1) The adenylation reaction involves nucleotide binding  to cleft 1 and NEDD8 binding to cleft 2; (2) the catalytic cysteine, facing NEDD8,  forms a thioester with NEDD8; (3) a second molecule of NEDD8 is adenylated; (4) occupation  of the nucleotide-binding pocket facilitates binding of E2 in cleft 1, promoting  transfer of the E1 thioester-linked Ublp to E2.	bind
3968	2	2286	6	10	NULL	0	NULL	NEDD8	GP		bind								cleft 2		NULL		NULL	NULL	NULL	NULL	gw70_nature_422_6929_330_s_139	12646924	(1) The adenylation reaction involves nucleotide binding  to cleft 1 and NEDD8 binding to cleft 2; (2) the catalytic cysteine, facing NEDD8,  forms a thioester with NEDD8; (3) a second molecule of NEDD8 is adenylated; (4) occupation  of the nucleotide-binding pocket facilitates binding of E2 in cleft 1, promoting  transfer of the E1 thioester-linked Ublp to E2.	bind
4615	3	2286	6	10	NULL	0	NULL	adenylation reaction	Process		involves					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_nature_422_6929_330_s_139	12646924	(1) The adenylation reaction involves nucleotide binding  to cleft 1 and NEDD8 binding to cleft 2; (2) the catalytic cysteine, facing NEDD8,  forms a thioester with NEDD8; (3) a second molecule of NEDD8 is adenylated; (4) occupation  of the nucleotide-binding pocket facilitates binding of E2 in cleft 1, promoting  transfer of the E1 thioester-linked Ublp to E2.	bind
4616	4	2286	6	10	NULL	0	NULL	adenylation reaction	Process		involves					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_nature_422_6929_330_s_139	12646924	(1) The adenylation reaction involves nucleotide binding  to cleft 1 and NEDD8 binding to cleft 2; (2) the catalytic cysteine, facing NEDD8,  forms a thioester with NEDD8; (3) a second molecule of NEDD8 is adenylated; (4) occupation  of the nucleotide-binding pocket facilitates binding of E2 in cleft 1, promoting  transfer of the E1 thioester-linked Ublp to E2.	bind
4617	5	2286	6	10	NULL	0	NULL	cysteine	AminoAcid	catalytic 	forms 					NEDD8	GP	thioester with			NULL		NULL	NULL	NULL	NULL	gw70_nature_422_6929_330_s_139	12646924	(1) The adenylation reaction involves nucleotide binding  to cleft 1 and NEDD8 binding to cleft 2; (2) the catalytic cysteine, facing NEDD8,  forms a thioester with NEDD8; (3) a second molecule of NEDD8 is adenylated; (4) occupation  of the nucleotide-binding pocket facilitates binding of E2 in cleft 1, promoting  transfer of the E1 thioester-linked Ublp to E2.	bind
4618	6	2286	6	10	NULL	0	NULL	E2	GP		bind								cleft 1		NULL		NULL	NULL	NULL	NULL	gw70_nature_422_6929_330_s_139	12646924	(1) The adenylation reaction involves nucleotide binding  to cleft 1 and NEDD8 binding to cleft 2; (2) the catalytic cysteine, facing NEDD8,  forms a thioester with NEDD8; (3) a second molecule of NEDD8 is adenylated; (4) occupation  of the nucleotide-binding pocket facilitates binding of E2 in cleft 1, promoting  transfer of the E1 thioester-linked Ublp to E2.	bind
4619	7	2286	6	10	NULL	0	NULL	NEDD8	GP		undergoes					adenylation	Process				NULL		NULL	NULL	NULL	NULL	gw70_nature_422_6929_330_s_139	12646924	(1) The adenylation reaction involves nucleotide binding  to cleft 1 and NEDD8 binding to cleft 2; (2) the catalytic cysteine, facing NEDD8,  forms a thioester with NEDD8; (3) a second molecule of NEDD8 is adenylated; (4) occupation  of the nucleotide-binding pocket facilitates binding of E2 in cleft 1, promoting  transfer of the E1 thioester-linked Ublp to E2.	bind
4621	10	2286	6	10	NULL	0	NULL	statement 8	Process		promote					statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw70_nature_422_6929_330_s_139	12646924	(1) The adenylation reaction involves nucleotide binding  to cleft 1 and NEDD8 binding to cleft 2; (2) the catalytic cysteine, facing NEDD8,  forms a thioester with NEDD8; (3) a second molecule of NEDD8 is adenylated; (4) occupation  of the nucleotide-binding pocket facilitates binding of E2 in cleft 1, promoting  transfer of the E1 thioester-linked Ublp to E2.	bind
46879	8	2286	6	10	NULL	0	NULL	nucleotide-binding pocket	NucleicAcid	occupation of 	faciliate					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_nature_422_6929_330_s_139	12646924	(1) The adenylation reaction involves nucleotide binding  to cleft 1 and NEDD8 binding to cleft 2; (2) the catalytic cysteine, facing NEDD8,  forms a thioester with NEDD8; (3) a second molecule of NEDD8 is adenylated; (4) occupation  of the nucleotide-binding pocket facilitates binding of E2 in cleft 1, promoting  transfer of the E1 thioester-linked Ublp to E2.	bind
46880	9	2286	6	10	NULL	0	NULL	Ublp	GP	E1 thioester-linked	is transfered to					E2	GP				NULL		NULL	NULL	NULL	NULL	gw70_nature_422_6929_330_s_139	12646924	(1) The adenylation reaction involves nucleotide binding  to cleft 1 and NEDD8 binding to cleft 2; (2) the catalytic cysteine, facing NEDD8,  forms a thioester with NEDD8; (3) a second molecule of NEDD8 is adenylated; (4) occupation  of the nucleotide-binding pocket facilitates binding of E2 in cleft 1, promoting  transfer of the E1 thioester-linked Ublp to E2.	bind
4118	2	2287	5	10	NULL	0	NULL	LRH-1	GP		differ from			coactivator binding surface 		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_devcell_5_1_1_s_35	12852843	(1) The coactivator binding surface in LRH-1 differs in its details from that found in prototypic agonist-bound nuclear receptors; as a result, coactivators may bind to LRH-1 by utilizing nontraditional receptor surfaces, or LRH-1 may use novel coactivators in place of the usual suspects.	bind
4119	3	2287	5	10	NULL	0	NULL	coactivators	GP		bind		may			LRH-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_5_1_1_s_35	12852843	(1) The coactivator binding surface in LRH-1 differs in its details from that found in prototypic agonist-bound nuclear receptors; as a result, coactivators may bind to LRH-1 by utilizing nontraditional receptor surfaces, or LRH-1 may use novel coactivators in place of the usual suspects.	bind
4120	4	2287	5	10	NULL	0	NULL	statement 2	Process		utilize					receptor surfaces	GP	nontraditional			NULL		NULL	NULL	NULL	NULL	gw60_devcell_5_1_1_s_35	12852843	(1) The coactivator binding surface in LRH-1 differs in its details from that found in prototypic agonist-bound nuclear receptors; as a result, coactivators may bind to LRH-1 by utilizing nontraditional receptor surfaces, or LRH-1 may use novel coactivators in place of the usual suspects.	bind
4121	5	2287	5	10	NULL	0	NULL	LRH-1	GP		use		may			coactivators	GP	novel			NULL		NULL	NULL	NULL	NULL	gw60_devcell_5_1_1_s_35	12852843	(1) The coactivator binding surface in LRH-1 differs in its details from that found in prototypic agonist-bound nuclear receptors; as a result, coactivators may bind to LRH-1 by utilizing nontraditional receptor surfaces, or LRH-1 may use novel coactivators in place of the usual suspects.	bind
4122	6	2287	5	10	NULL	0	NULL	statement 2	NULL		results in	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_devcell_5_1_1_s_35	12852843	(1) The coactivator binding surface in LRH-1 differs in its details from that found in prototypic agonist-bound nuclear receptors; as a result, coactivators may bind to LRH-1 by utilizing nontraditional receptor surfaces, or LRH-1 may use novel coactivators in place of the usual suspects.	bind
4123	7	2287	5	10	NULL	0	NULL	statement 2	NULL		results in	NULL				statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw60_devcell_5_1_1_s_35	12852843	(1) The coactivator binding surface in LRH-1 differs in its details from that found in prototypic agonist-bound nuclear receptors; as a result, coactivators may bind to LRH-1 by utilizing nontraditional receptor surfaces, or LRH-1 may use novel coactivators in place of the usual suspects.	bind
5258	8	2287	5	10	NULL	0	NULL	statement 6	NULL		is an alternative to	NULL				statement 7	NULL				NULL		NULL	NULL	NULL	NULL	gw60_devcell_5_1_1_s_35	12852843	(1) The coactivator binding surface in LRH-1 differs in its details from that found in prototypic agonist-bound nuclear receptors; as a result, coactivators may bind to LRH-1 by utilizing nontraditional receptor surfaces, or LRH-1 may use novel coactivators in place of the usual suspects.	bind
46426	1	2287	5	10	NULL	0	NULL	prototypic agonist	Chemical		bind					nuclear receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_5_1_1_s_35	12852843	(1) The coactivator binding surface in LRH-1 differs in its details from that found in prototypic agonist-bound nuclear receptors; as a result, coactivators may bind to LRH-1 by utilizing nontraditional receptor surfaces, or LRH-1 may use novel coactivators in place of the usual suspects.	bind
4622	1	2287	6	10	NULL	0	NULL	coactivator	GP		bind		may			LRH-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_5_1_1_s_35	12852843	(1) The coactivator binding surface in LRH-1 differs in its details from that found in prototypic agonist-bound nuclear receptors; as a result, coactivators may bind to LRH-1 by utilizing nontraditional receptor surfaces, or LRH-1 may use novel coactivators in place of the usual suspects.	bind
4623	2	2287	6	10	NULL	0	NULL	statement 1	Process		utilize					receptor surface	GP	nontraditional			NULL		NULL	NULL	NULL	NULL	gw60_devcell_5_1_1_s_35	12852843	(1) The coactivator binding surface in LRH-1 differs in its details from that found in prototypic agonist-bound nuclear receptors; as a result, coactivators may bind to LRH-1 by utilizing nontraditional receptor surfaces, or LRH-1 may use novel coactivators in place of the usual suspects.	bind
4989	4	2287	6	10	NULL	0	NULL	LRH-1	GP		differ from			coactivator binding surface 		statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_devcell_5_1_1_s_35	12852843	(1) The coactivator binding surface in LRH-1 differs in its details from that found in prototypic agonist-bound nuclear receptors; as a result, coactivators may bind to LRH-1 by utilizing nontraditional receptor surfaces, or LRH-1 may use novel coactivators in place of the usual suspects.	bind
4990	5	2287	6	10	NULL	0	NULL	LRH-1	GP		use		may			coactivators	GP	novel			NULL		NULL	NULL	NULL	NULL	gw60_devcell_5_1_1_s_35	12852843	(1) The coactivator binding surface in LRH-1 differs in its details from that found in prototypic agonist-bound nuclear receptors; as a result, coactivators may bind to LRH-1 by utilizing nontraditional receptor surfaces, or LRH-1 may use novel coactivators in place of the usual suspects.	bind
4991	6	2287	6	10	NULL	0	NULL	statement 4	Process		results in					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_devcell_5_1_1_s_35	12852843	(1) The coactivator binding surface in LRH-1 differs in its details from that found in prototypic agonist-bound nuclear receptors; as a result, coactivators may bind to LRH-1 by utilizing nontraditional receptor surfaces, or LRH-1 may use novel coactivators in place of the usual suspects.	bind
4992	7	2287	6	10	NULL	0	NULL	statement 4	Process		results in					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_devcell_5_1_1_s_35	12852843	(1) The coactivator binding surface in LRH-1 differs in its details from that found in prototypic agonist-bound nuclear receptors; as a result, coactivators may bind to LRH-1 by utilizing nontraditional receptor surfaces, or LRH-1 may use novel coactivators in place of the usual suspects.	bind
4993	8	2287	6	10	NULL	0	NULL	statement 6	Process		is an alternative to					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_devcell_5_1_1_s_35	12852843	(1) The coactivator binding surface in LRH-1 differs in its details from that found in prototypic agonist-bound nuclear receptors; as a result, coactivators may bind to LRH-1 by utilizing nontraditional receptor surfaces, or LRH-1 may use novel coactivators in place of the usual suspects.	bind
46427	3	2287	6	10	NULL	0	NULL	prototypic agonist	Chemical		bind					nuclear receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_5_1_1_s_35	12852843	(1) The coactivator binding surface in LRH-1 differs in its details from that found in prototypic agonist-bound nuclear receptors; as a result, coactivators may bind to LRH-1 by utilizing nontraditional receptor surfaces, or LRH-1 may use novel coactivators in place of the usual suspects.	bind
4124	1	2288	5	10	NULL	0	NULL	import substrate	GP		bind					importin-alpha/beta heterodimer	GP		NLS binding site		NULL		NULL	NULL	NULL	NULL	gw60_embo_17_10_2721_s_59	9582265	(1) The initial, cytoplasmic event in NLS-dependent import is the binding of the import substrate to the importin-alpha/beta heterodimer, where the importin-alpha subunit provides the NLS binding site.	bind
4125	2	2288	5	10	NULL	0	NULL	importin-alpha subunit	GP		provide								NLS binding site		NULL		NULL	NULL	NULL	NULL	gw60_embo_17_10_2721_s_59	9582265	(1) The initial, cytoplasmic event in NLS-dependent import is the binding of the import substrate to the importin-alpha/beta heterodimer, where the importin-alpha subunit provides the NLS binding site.	bind
4126	3	2288	5	10	NULL	0	NULL	NLS-dependent import	Process	initial, cytoplasmic event in	involves					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_10_2721_s_59	9582265	(1) The initial, cytoplasmic event in NLS-dependent import is the binding of the import substrate to the importin-alpha/beta heterodimer, where the importin-alpha subunit provides the NLS binding site.	bind
3969	1	2288	6	10	NULL	0	NULL	import substrate	GP		bind					 importin-alpha/beta heterodimer	GP		NLS binding site		NULL		NULL	NULL	NULL	NULL	gw60_embo_17_10_2721_s_59	9582265	(1) The initial, cytoplasmic event in NLS-dependent import is the binding of the import substrate to the importin-alpha/beta heterodimer, where the importin-alpha subunit provides the NLS binding site.	bind
3970	2	2288	6	10	NULL	0	NULL	importin-alpha subunit	GP		provides								NLS binding site		NULL		NULL	NULL	NULL	NULL	gw60_embo_17_10_2721_s_59	9582265	(1) The initial, cytoplasmic event in NLS-dependent import is the binding of the import substrate to the importin-alpha/beta heterodimer, where the importin-alpha subunit provides the NLS binding site.	bind
52991	3	2288	6	10	NULL	0	NULL	NLS-dependent import	Process	initial, cytoplasmic event in	involves					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_10_2721_s_59	9582265	(1) The initial, cytoplasmic event in NLS-dependent import is the binding of the import substrate to the importin-alpha/beta heterodimer, where the importin-alpha subunit provides the NLS binding site.	bind
4127	1	2289	5	10	NULL	0	NULL	MS2 peptide	GP		bind								fourth Ig-like domain		NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_18_9_3460_s_150	9547253	(1) The peptide MS2, which binds to the fourth Ig-like domain, reduced the magnitude of LTP by a constant amount, from the beginning to the end of the recording period after TBS, but only if it was present during TBS.	bind
4128	2	2289	5	10	NULL	0	NULL	statement 1	Process		reduced					LTP	Process	magnitude of			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_18_9_3460_s_150	9547253	(1) The peptide MS2, which binds to the fourth Ig-like domain, reduced the magnitude of LTP by a constant amount, from the beginning to the end of the recording period after TBS, but only if it was present during TBS.	bind
3971	1	2289	6	10	NULL	0	NULL	MS2 peptide	GP		bind								fourth Ig-like domain		NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_18_9_3460_s_150	9547253	(1) The peptide MS2, which binds to the fourth Ig-like domain, reduced the magnitude of LTP by a constant amount, from the beginning to the end of the recording period after TBS, but only if it was present during TBS.	bind
3972	2	2289	6	10	NULL	0	NULL	MS2 peptide	GP		reduces					LTP	Process	magnitude of			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_18_9_3460_s_150	9547253	(1) The peptide MS2, which binds to the fourth Ig-like domain, reduced the magnitude of LTP by a constant amount, from the beginning to the end of the recording period after TBS, but only if it was present during TBS.	bind
4129	1	2291	5	10	NULL	0	NULL	synuclein	GP		bind					BAD	GP				NULL	cytoplasm	NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
4131	2	2291	5	10	NULL	0	NULL	BAD	GP		translocated to					mitochondria	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
4132	3	2291	5	10	NULL	0	NULL	statement 1	Process		prevent					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
4133	5	2291	5	10	NULL	0	NULL	BAD	GP		induce					cytochrome c	GP	release			NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
4134	6	2291	5	10	NULL	0	NULL	MPP+	Chemical	exposure	inhibit					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
4135	7	2291	5	10	NULL	0	NULL	cytochrome c	GP		mediate					caspase-3	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
4136	8	2291	5	10	NULL	0	NULL	MPP+	Chemical	exposure of	block		subsequently			statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
4137	9	2291	5	10	NULL	0	NULL	caspase-3	GP		mediate					PKC	GP	 proteolytic cleavage			NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
4138	10	2291	5	10	NULL	0	NULL	MPP+	Chemical	exposure	attenuate					statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
4139	11	2291	5	10	NULL	0	NULL	synuclein	GP		bind					PKC	GP				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
4140	12	2291	5	10	NULL	0	NULL	statement 11	Process		prevent					PKC	GP	proteolytic cleavage of			NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
4141	13	2291	5	10	NULL	0	NULL	statement 12	Process		attenuate		significantly			DNA fragmentation	Process				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
4142	14	2291	5	10	NULL	0	NULL	statement 12	Process		attenuate		significantly			cellular apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
46428	4	2291	5	10	NULL	0	NULL	statement 1	Process		occurs upon					MPP+	Chemical	exposure to			NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
46429	15	2291	5	10	NULL	0	NULL	BAD	GP		is a type of					 pro-apoptotic factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
46430	16	2291	5	10	NULL	0	NULL	PKC	GP		is a type of					pro-apoptotic kinase	GP				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
4624	1	2291	6	10	NULL	0	NULL	synuclein	GP		bind					BAD	GP				NULL	cytoplasm	NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
4994	2	2291	6	10	NULL	0	NULL	statement 1	Process		occurs upon 					MPP+	Chemical	exposure of			NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
4995	3	2291	6	10	NULL	0	NULL	BAD	GP		induces					cytochrome c	GP	release of			NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
4996	4	2291	6	10	NULL	0	NULL	MPP+	Chemical	exposure to	inhibits					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
4997	5	2291	6	10	NULL	0	NULL	cytochrome c	GP		mediates					caspase-3	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
4998	6	2291	6	10	NULL	0	NULL	MPP+	Chemical	exposure to	blocks					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
4999	7	2291	6	10	NULL	0	NULL	caspase-3	GP		mediates					PKC	GP	proteolytic cleavage of			NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
5000	8	2291	6	10	NULL	0	NULL	MPP+	Chemical	exposure to	attenuates					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
5001	9	2291	6	10	NULL	0	NULL	synuclein	GP		bind					PKC	GP				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
5002	10	2291	6	10	NULL	0	NULL	statement 9	Process		prevents					PKC	GP	proteolytic cleavage of			NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
5003	11	2291	6	10	NULL	0	NULL	statement 10	Process		attenuates		significantly			DNA fragmentation	Process				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
5004	12	2291	6	10	NULL	0	NULL	statement 10	Process		attenuates		significantly			cellular apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
46433	13	2291	6	10	NULL	0	NULL	BAD	GP		translocates to					mitochondria	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
46434	14	2291	6	10	NULL	0	NULL	statement 1	Process		prevents					statement 13	Process				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
46436	15	2291	6	10	NULL	0	NULL	BAD	GP		is a type of					pro-apoptotic factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
46437	16	2291	6	10	NULL	0	NULL	PKC	GP		is a type of					pro-apoptotic kinase	GP				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_139_1_137_s_367	15978696	(1) Upon exposure to MPP+,  -synuclein binds to the pro-apoptotic factor BAD in the cytoplasm and prevents  its translocation to the mitochondria; (2) BAD-induced cytochrome  c release is inhibited; (3) cytochrome  c-mediated activation of caspase-3 is subsequently blocked; (4) caspase-3-mediated  proteolytic cleavage of PKC  is attenuated; (5)  -synuclein also binds to the pro-apoptotic  kinase PKC  and (6) prevents proteolytic cleavage of PKC  which significantly attenuates  (7) DNA fragmentation and cellular apoptosis.	bind
4144	1	2293	5	10	NULL	0	NULL	protein b1	GP		bind					protein bn	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_18_5945_s_81	16237128	(1) where  P( b1| bn) is the probability of finding a protein bound right next to another one that is already bound to DNA ( ).  b1| bn denotes the protein  b1 binding to the protein  bn:	bind
4275	2	2293	5	10	NULL	0	NULL	b1| bn	GP		denotes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_18_5945_s_81	16237128	(1) where  P( b1| bn) is the probability of finding a protein bound right next to another one that is already bound to DNA ( ).  b1| bn denotes the protein  b1 binding to the protein  bn:	bind
3975	1	2293	6	10	NULL	0	NULL	protein b1	GP		bind					protein bn	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_18_5945_s_81	16237128	(1) where  P( b1| bn) is the probability of finding a protein bound right next to another one that is already bound to DNA ( ).  b1| bn denotes the protein  b1 binding to the protein  bn:	bind
3976	2	2293	6	10	NULL	0	NULL	statement 1	Process		denotes					 b1| bn	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_18_5945_s_81	16237128	(1) where  P( b1| bn) is the probability of finding a protein bound right next to another one that is already bound to DNA ( ).  b1| bn denotes the protein  b1 binding to the protein  bn:	bind
4145	1	2294	5	10	NULL	0	NULL	cAMP	NucleicAcid		bind					PKA	GP				NULL	lateral region of the caudate-putamen and the parietal cortex	NULL	NULL	NULL	NULL	gw60_neuroscience_94_2_361_s_218	10579200	(1) Within 3 h of MCA occlusion, there was a significant reduction in cAMP binding to PKA in the lateral region of the caudate-putamen and the parietal cortex.	bind
4146	2	2294	5	10	NULL	0	NULL	MCA 	OrganismPart	occlusion of	reduce		significantly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_94_2_361_s_218	10579200	(1) Within 3 h of MCA occlusion, there was a significant reduction in cAMP binding to PKA in the lateral region of the caudate-putamen and the parietal cortex.	bind
4030	1	2294	6	10	NULL	0	NULL	cAMP	NucleicAcid		bind					PKA	GP				NULL	lateral region of the caudate-putamen and the parietal cortex	NULL	NULL	NULL	NULL	gw60_neuroscience_94_2_361_s_218	10579200	(1) Within 3 h of MCA occlusion, there was a significant reduction in cAMP binding to PKA in the lateral region of the caudate-putamen and the parietal cortex.	bind
4031	2	2294	6	10	NULL	0	NULL	MCA	OrganismPart	occlusion of	reduce		significantly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_94_2_361_s_218	10579200	(1) Within 3 h of MCA occlusion, there was a significant reduction in cAMP binding to PKA in the lateral region of the caudate-putamen and the parietal cortex.	bind
4175	1	2295	5	10	NULL	0	NULL	ATP-actin	GP		bind					profilin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_4_453_s_88	12600310	(10) Profilin catalyzes the exchange of ADP for ATP (turning the subunits white), returning subunits to (11) the pool of ATP-actin bound to profilin, ready to elongate barbed ends as they become available.	bind
4176	2	2295	5	10	NULL	0	NULL	ADP	Chemical		exchange for					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_4_453_s_88	12600310	(10) Profilin catalyzes the exchange of ADP for ATP (turning the subunits white), returning subunits to (11) the pool of ATP-actin bound to profilin, ready to elongate barbed ends as they become available.	bind
4177	3	2295	5	10	NULL	0	NULL	profilin	GP		catalyze					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_4_453_s_88	12600310	(10) Profilin catalyzes the exchange of ADP for ATP (turning the subunits white), returning subunits to (11) the pool of ATP-actin bound to profilin, ready to elongate barbed ends as they become available.	bind
4051	1	2295	6	10	NULL	0	NULL	ATP-actin	GP		bind					profilin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_4_453_s_88	12600310	(10) Profilin catalyzes the exchange of ADP for ATP (turning the subunits white), returning subunits to (11) the pool of ATP-actin bound to profilin, ready to elongate barbed ends as they become available.	bind
4630	2	2295	6	10	NULL	0	NULL	ADP	Chemical		exchange for					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_4_453_s_88	12600310	(10) Profilin catalyzes the exchange of ADP for ATP (turning the subunits white), returning subunits to (11) the pool of ATP-actin bound to profilin, ready to elongate barbed ends as they become available.	bind
4631	3	2295	6	10	NULL	0	NULL	profilin	GP		catalyzes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_4_453_s_88	12600310	(10) Profilin catalyzes the exchange of ADP for ATP (turning the subunits white), returning subunits to (11) the pool of ATP-actin bound to profilin, ready to elongate barbed ends as they become available.	bind
4179	1	2296	5	10	NULL	0	NULL	(125)I-C5	GP		bind		reversibly			C6	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_274_45_10542204_s_7	10542204	(125)I-C5 binds reversibly  to C6 in an ionic strength-dependent fashion, but (125)I-C5 binds only  weakly to C6des-FIMs and not at all to C6des-CCP/FIMs.	bind
4180	2	2296	5	10	NULL	0	NULL	statement 1	Process		is dependent on					ionic strength	QuantityOrMeasure				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_274_45_10542204_s_7	10542204	(125)I-C5 binds reversibly  to C6 in an ionic strength-dependent fashion, but (125)I-C5 binds only  weakly to C6des-FIMs and not at all to C6des-CCP/FIMs.	bind
4181	3	2296	5	10	NULL	0	NULL	(125)I-C5	GP		bind		weakly			C6	GP		des-FIMs		NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_274_45_10542204_s_7	10542204	(125)I-C5 binds reversibly  to C6 in an ionic strength-dependent fashion, but (125)I-C5 binds only  weakly to C6des-FIMs and not at all to C6des-CCP/FIMs.	bind
4182	4	2296	5	10	NULL	0	NULL	(125)I-C5	GP		does not bind					C6	GP		des-CCP/FIMs		NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_274_45_10542204_s_7	10542204	(125)I-C5 binds reversibly  to C6 in an ionic strength-dependent fashion, but (125)I-C5 binds only  weakly to C6des-FIMs and not at all to C6des-CCP/FIMs.	bind
4052	1	2296	6	10	NULL	0	NULL	I-C5	GP		bind		reversibly			C6	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_274_45_10542204_s_7	10542204	(125)I-C5 binds reversibly  to C6 in an ionic strength-dependent fashion, but (125)I-C5 binds only  weakly to C6des-FIMs and not at all to C6des-CCP/FIMs.	bind
4053	2	2296	6	10	NULL	0	NULL	statement 1	Process		is dependent on					ionic strength	QuantityOrMeasure				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_274_45_10542204_s_7	10542204	(125)I-C5 binds reversibly  to C6 in an ionic strength-dependent fashion, but (125)I-C5 binds only  weakly to C6des-FIMs and not at all to C6des-CCP/FIMs.	bind
4054	3	2296	6	10	NULL	0	NULL	I-C5	GP		bind		weakly			C6	GP		des-FIMs		NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_274_45_10542204_s_7	10542204	(125)I-C5 binds reversibly  to C6 in an ionic strength-dependent fashion, but (125)I-C5 binds only  weakly to C6des-FIMs and not at all to C6des-CCP/FIMs.	bind
4055	4	2296	6	10	NULL	0	NULL	I-C5	GP		does not bind					C6	GP		des-CCP/FIMs		NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_274_45_10542204_s_7	10542204	(125)I-C5 binds reversibly  to C6 in an ionic strength-dependent fashion, but (125)I-C5 binds only  weakly to C6des-FIMs and not at all to C6des-CCP/FIMs.	bind
4183	1	2297	5	10	NULL	0	NULL	Cry1Ac	GP	(125)I-labeled	bind		specifically			brush border membrane vesicles	CellComponent	E. insulana			NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_appl-environ-microbiol_72_1_16391075_s_12	16391075	(125)I-labeled Cry1Ac and Cry1Ab and biotinylated Cry1Ba,  Cry1Ia, and Cry9Ca showed specific binding to the brush border membrane  vesicles from E. insulana.	bind
4184	2	2297	5	10	NULL	0	NULL	Cry1Ab	GP	(125)I-labeled	bind		specifically			brush border membrane vesicles	CellComponent	E. insulana			NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_appl-environ-microbiol_72_1_16391075_s_12	16391075	(125)I-labeled Cry1Ac and Cry1Ab and biotinylated Cry1Ba,  Cry1Ia, and Cry9Ca showed specific binding to the brush border membrane  vesicles from E. insulana.	bind
4185	3	2297	5	10	NULL	0	NULL	Cry1Ba	GP	biotinylated	bind		specifically			brush border membrane vesicles	CellComponent	E. insulana			NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_appl-environ-microbiol_72_1_16391075_s_12	16391075	(125)I-labeled Cry1Ac and Cry1Ab and biotinylated Cry1Ba,  Cry1Ia, and Cry9Ca showed specific binding to the brush border membrane  vesicles from E. insulana.	bind
4186	4	2297	5	10	NULL	0	NULL	Cry1Ia	GP	biotinylated	bind		specifically			brush border membrane vesicles	CellComponent	E. insulana			NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_appl-environ-microbiol_72_1_16391075_s_12	16391075	(125)I-labeled Cry1Ac and Cry1Ab and biotinylated Cry1Ba,  Cry1Ia, and Cry9Ca showed specific binding to the brush border membrane  vesicles from E. insulana.	bind
4187	5	2297	5	10	NULL	0	NULL	Cry9Ca	GP	biotinylated	bind		specifically			brush border membrane vesicles	CellComponent	E. insulana			NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_appl-environ-microbiol_72_1_16391075_s_12	16391075	(125)I-labeled Cry1Ac and Cry1Ab and biotinylated Cry1Ba,  Cry1Ia, and Cry9Ca showed specific binding to the brush border membrane  vesicles from E. insulana.	bind
4056	1	2297	6	10	NULL	0	NULL	Cry1Ac	GP	(125)I-labeled	bind		specifically			brush border membrane vesicles	CellComponent	E. insulana  			NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_appl-environ-microbiol_72_1_16391075_s_12	16391075	(125)I-labeled Cry1Ac and Cry1Ab and biotinylated Cry1Ba,  Cry1Ia, and Cry9Ca showed specific binding to the brush border membrane  vesicles from E. insulana.	bind
4057	2	2297	6	10	NULL	0	NULL	Cry1Ab	GP	(125)I-labeled	bind		specifically			brush border membrane vesicles	CellComponent	E. insulana			NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_appl-environ-microbiol_72_1_16391075_s_12	16391075	(125)I-labeled Cry1Ac and Cry1Ab and biotinylated Cry1Ba,  Cry1Ia, and Cry9Ca showed specific binding to the brush border membrane  vesicles from E. insulana.	bind
4058	3	2297	6	10	NULL	0	NULL	Cry1Ba	GP	biotinylated	bind		specifically			brush border membrane vesicles	CellComponent	E. insulana			NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_appl-environ-microbiol_72_1_16391075_s_12	16391075	(125)I-labeled Cry1Ac and Cry1Ab and biotinylated Cry1Ba,  Cry1Ia, and Cry9Ca showed specific binding to the brush border membrane  vesicles from E. insulana.	bind
4059	4	2297	6	10	NULL	0	NULL	Cry1Ia	GP	biotinylated	bind		specifically			brush border membrane vesicles	CellComponent	E. insulana  			NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_appl-environ-microbiol_72_1_16391075_s_12	16391075	(125)I-labeled Cry1Ac and Cry1Ab and biotinylated Cry1Ba,  Cry1Ia, and Cry9Ca showed specific binding to the brush border membrane  vesicles from E. insulana.	bind
4060	5	2297	6	10	NULL	0	NULL	Cry9Ca	GP	biotinylated	bind		specifically			brush border membrane vesicles	CellComponent	E. insulana			NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_appl-environ-microbiol_72_1_16391075_s_12	16391075	(125)I-labeled Cry1Ac and Cry1Ab and biotinylated Cry1Ba,  Cry1Ia, and Cry9Ca showed specific binding to the brush border membrane  vesicles from E. insulana.	bind
4188	1	2298	5	10	NULL	0	NULL	dopamine	Chemical		bind					striatal D-2 site	OrganismPart	rat			NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_128_4_881_s_263	10556922	(1982) [3]-dopamine binding to rat striatal D-2 and D-3 sites: enhancement by magnesium and inhibition by guanine nucleotides and sodium.	bind
4189	2	2298	5	10	NULL	0	NULL	dopamine	Chemical		bind					striatal D-3 site	OrganismPart	rat			NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_128_4_881_s_263	10556922	(1982) [3]-dopamine binding to rat striatal D-2 and D-3 sites: enhancement by magnesium and inhibition by guanine nucleotides and sodium.	bind
5259	3	2298	5	10	NULL	0	NULL	magnesium	Chemical		enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_128_4_881_s_263	10556922	(1982) [3]-dopamine binding to rat striatal D-2 and D-3 sites: enhancement by magnesium and inhibition by guanine nucleotides and sodium.	bind
5260	4	2298	5	10	NULL	0	NULL	magnesium	Chemical		enhance					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_128_4_881_s_263	10556922	(1982) [3]-dopamine binding to rat striatal D-2 and D-3 sites: enhancement by magnesium and inhibition by guanine nucleotides and sodium.	bind
5261	5	2298	5	10	NULL	0	NULL	guanine nucleotides	NucleicAcid		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_128_4_881_s_263	10556922	(1982) [3]-dopamine binding to rat striatal D-2 and D-3 sites: enhancement by magnesium and inhibition by guanine nucleotides and sodium.	bind
5262	6	2298	5	10	NULL	0	NULL	guanine nucleotides	NucleicAcid		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_128_4_881_s_263	10556922	(1982) [3]-dopamine binding to rat striatal D-2 and D-3 sites: enhancement by magnesium and inhibition by guanine nucleotides and sodium.	bind
5263	7	2298	5	10	NULL	0	NULL	sodium	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_128_4_881_s_263	10556922	(1982) [3]-dopamine binding to rat striatal D-2 and D-3 sites: enhancement by magnesium and inhibition by guanine nucleotides and sodium.	bind
5264	8	2298	5	10	NULL	0	NULL	sodium	Chemical		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_128_4_881_s_263	10556922	(1982) [3]-dopamine binding to rat striatal D-2 and D-3 sites: enhancement by magnesium and inhibition by guanine nucleotides and sodium.	bind
4061	1	2298	6	10	NULL	0	NULL	dopamine	Chemical		bind					striatal D-2 site	OrganismPart	rat			NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_128_4_881_s_263	10556922	(1982) [3]-dopamine binding to rat striatal D-2 and D-3 sites: enhancement by magnesium and inhibition by guanine nucleotides and sodium.	bind
4062	2	2298	6	10	NULL	0	NULL	dopamine	Chemical		bind					striatal D-3 site	OrganismPart	rat			NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_128_4_881_s_263	10556922	(1982) [3]-dopamine binding to rat striatal D-2 and D-3 sites: enhancement by magnesium and inhibition by guanine nucleotides and sodium.	bind
4063	3	2298	6	10	NULL	0	NULL	magnesium	Chemical		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_128_4_881_s_263	10556922	(1982) [3]-dopamine binding to rat striatal D-2 and D-3 sites: enhancement by magnesium and inhibition by guanine nucleotides and sodium.	bind
4064	4	2298	6	10	NULL	0	NULL	magnesium	Chemical		enhances					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_128_4_881_s_263	10556922	(1982) [3]-dopamine binding to rat striatal D-2 and D-3 sites: enhancement by magnesium and inhibition by guanine nucleotides and sodium.	bind
4065	5	2298	6	10	NULL	0	NULL	guanine nucleotides	NucleicAcid		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_128_4_881_s_263	10556922	(1982) [3]-dopamine binding to rat striatal D-2 and D-3 sites: enhancement by magnesium and inhibition by guanine nucleotides and sodium.	bind
4066	6	2298	6	10	NULL	0	NULL	guanine nucleotides	NucleicAcid		inhibits					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_128_4_881_s_263	10556922	(1982) [3]-dopamine binding to rat striatal D-2 and D-3 sites: enhancement by magnesium and inhibition by guanine nucleotides and sodium.	bind
4067	7	2298	6	10	NULL	0	NULL	sodium	Chemical		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_128_4_881_s_263	10556922	(1982) [3]-dopamine binding to rat striatal D-2 and D-3 sites: enhancement by magnesium and inhibition by guanine nucleotides and sodium.	bind
4068	8	2298	6	10	NULL	0	NULL	sodium	Chemical		inhibits					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_128_4_881_s_263	10556922	(1982) [3]-dopamine binding to rat striatal D-2 and D-3 sites: enhancement by magnesium and inhibition by guanine nucleotides and sodium.	bind
4190	1	2299	5	10	NULL	0	NULL	Acyl-CoA	GP		bind					FadR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33652_s_358	9837950	(1991)  J. Biol. Chem.  266, 23824-23828 [Abstract]         aman, N.    (1996)   tudies on Acyl-CoA Binding to the Transcription Factor FadR, Ph.D. dissertation, University of Tennessee, Memphis	bind
52992	2	2299	5	10	NULL	0	NULL	FadR	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33652_s_358	9837950	(1991)  J. Biol. Chem.  266, 23824-23828 [Abstract]         aman, N.    (1996)   tudies on Acyl-CoA Binding to the Transcription Factor FadR, Ph.D. dissertation, University of Tennessee, Memphis	bind
4069	1	2299	6	10	NULL	0	NULL	Acyl-CoA	GP		bind					FadR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33652_s_358	9837950	(1991)  J. Biol. Chem.  266, 23824-23828 [Abstract]         aman, N.    (1996)   tudies on Acyl-CoA Binding to the Transcription Factor FadR, Ph.D. dissertation, University of Tennessee, Memphis	bind
52993	2	2299	6	10	NULL	0	NULL	FadR	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33652_s_358	9837950	(1991)  J. Biol. Chem.  266, 23824-23828 [Abstract]         aman, N.    (1996)   tudies on Acyl-CoA Binding to the Transcription Factor FadR, Ph.D. dissertation, University of Tennessee, Memphis	bind
4191	1	2300	5	10	NULL	0	NULL	P-glycoprotein	GP		contains								azidopine binding site		NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiolrev_21_1_55_s_961	9299702	(1992) Characterization of the azidopine and vinblastine binding site of P-glycoprotein.	bind
4192	2	2300	5	10	NULL	0	NULL	P-glycoprotein	GP		contains								vinblastine binding site		NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiolrev_21_1_55_s_961	9299702	(1992) Characterization of the azidopine and vinblastine binding site of P-glycoprotein.	bind
4632	1	2300	6	10	NULL	0	NULL	P-glycoprotein	GP		contains								azidopine binding site		NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiolrev_21_1_55_s_961	9299702	(1992) Characterization of the azidopine and vinblastine binding site of P-glycoprotein.	bind
4633	2	2300	6	10	NULL	0	NULL	P-glycoprotein	GP		contains								 vinblastine binding site		NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiolrev_21_1_55_s_961	9299702	(1992) Characterization of the azidopine and vinblastine binding site of P-glycoprotein.	bind
4193	1	2301	5	10	NULL	0	NULL	casein kinase II	GP		phosphorylate					mUBF	GP		C-terminal hyperacidic tail		NULL		NULL	NULL	NULL	NULL	gw60_embo_17_13_3692_s_462	9649439	(1992) The nucleolar transcription factor mUBF is phosphorylated by casein kinase II in the C-terminal hyperacidic tail which is essential for transactivation.	bind
4194	2	2301	5	10	NULL	0	NULL	mUBF	GP		is essential for			C-terminal hyperacidic tail		transactivation	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_13_3692_s_462	9649439	(1992) The nucleolar transcription factor mUBF is phosphorylated by casein kinase II in the C-terminal hyperacidic tail which is essential for transactivation.	bind
46457	3	2301	5	10	NULL	0	NULL	mUBF	GP		is a type of					nucleolar transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_13_3692_s_462	9649439	(1992) The nucleolar transcription factor mUBF is phosphorylated by casein kinase II in the C-terminal hyperacidic tail which is essential for transactivation.	bind
4070	1	2301	6	10	NULL	0	NULL	casein kinase II	GP		phosphorylates					mUBF	GP		C-terminal hyperacidic tail		NULL		NULL	NULL	NULL	NULL	gw60_embo_17_13_3692_s_462	9649439	(1992) The nucleolar transcription factor mUBF is phosphorylated by casein kinase II in the C-terminal hyperacidic tail which is essential for transactivation.	bind
4071	2	2301	6	10	NULL	0	NULL	mUBF	GP		is essential for			C-terminal hyperacidic tail		transactivation	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_13_3692_s_462	9649439	(1992) The nucleolar transcription factor mUBF is phosphorylated by casein kinase II in the C-terminal hyperacidic tail which is essential for transactivation.	bind
46458	3	2301	6	10	NULL	0	NULL	mUBF	GP		is a type of					nucleolar transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_13_3692_s_462	9649439	(1992) The nucleolar transcription factor mUBF is phosphorylated by casein kinase II in the C-terminal hyperacidic tail which is essential for transactivation.	bind
4195	1	2302	5	10	NULL	0	NULL	collagen	GP		bind					NG7C	Organism				NULL		NULL	NULL	NULL	NULL	gw60_femsimmunolmedmic_19_3_247_s_213	9453395	(1993) Collagen binding to  Escherichia coli strain NG7C.	bind
61101	2	2302	5	10	NULL	0	NULL	NG7C	Organism		is a strain of					Escherichia coli	Organism				NULL		NULL	NULL	NULL	NULL	gw60_femsimmunolmedmic_19_3_247_s_213	9453395	(1993) Collagen binding to  Escherichia coli strain NG7C.	bind
4073	1	2302	6	10	NULL	0	NULL	Collagen	GP		bind					 NG7C	Organism				NULL		NULL	NULL	NULL	NULL	gw60_femsimmunolmedmic_19_3_247_s_213	9453395	(1993) Collagen binding to  Escherichia coli strain NG7C.	bind
61102	2	2302	6	10	NULL	0	NULL	NG7C	Organism		is a strain of					Escherichia coli	Organism				NULL		0	NULL	NULL	NULL	gw60_femsimmunolmedmic_19_3_247_s_213	9453395	(1993) Collagen binding to  Escherichia coli strain NG7C.	bind
4196	1	2303	5	10	NULL	0	NULL	tissue plasminogen activator	GP		bind					endothelial cell membrane receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_1_146_s_233	8550827	(1993) Homocysteine-induced modulation of tissue plasminogen activator binding to its endothelial cell membrane receptor.	bind
4197	2	2303	5	10	NULL	0	NULL	homocysteine	AminoAcid		induce					statement 1	Process	modulation of			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_1_146_s_233	8550827	(1993) Homocysteine-induced modulation of tissue plasminogen activator binding to its endothelial cell membrane receptor.	bind
4074	1	2303	6	10	NULL	0	NULL	tissue plasminogen activator	GP		bind					endothelial cell membrane receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_1_146_s_233	8550827	(1993) Homocysteine-induced modulation of tissue plasminogen activator binding to its endothelial cell membrane receptor.	bind
4075	2	2303	6	10	NULL	0	NULL	Homocysteine	AminoAcid		induce					statement 1	Process	modulation  of			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_1_146_s_233	8550827	(1993) Homocysteine-induced modulation of tissue plasminogen activator binding to its endothelial cell membrane receptor.	bind
4198	1	2304	5	10	NULL	0	NULL	NAD+	Chemical		bind					TrkA	GP	Escherichia coli 			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_13_3491_s_184	9642210	(1993) NAD+ binding to the  Escherichia coli K+-uptake protein TrkA and sequence similarity between TrkA and domains of a family of dehydrogenases suggest a role of NAD+ in bacterial transport.	bind
4199	2	2304	5	10	NULL	0	NULL	TrkA	GP	sequence 	is similar to					dehydrogenases	GP	a family of 	domains of		NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_13_3491_s_184	9642210	(1993) NAD+ binding to the  Escherichia coli K+-uptake protein TrkA and sequence similarity between TrkA and domains of a family of dehydrogenases suggest a role of NAD+ in bacterial transport.	bind
4200	3	2304	5	10	NULL	0	NULL	NAD+	Chemical		is required for					bacterial transport	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_13_3491_s_184	9642210	(1993) NAD+ binding to the  Escherichia coli K+-uptake protein TrkA and sequence similarity between TrkA and domains of a family of dehydrogenases suggest a role of NAD+ in bacterial transport.	bind
4201	4	2304	5	10	NULL	0	NULL	statement 1	Process		suggest					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_13_3491_s_184	9642210	(1993) NAD+ binding to the  Escherichia coli K+-uptake protein TrkA and sequence similarity between TrkA and domains of a family of dehydrogenases suggest a role of NAD+ in bacterial transport.	bind
4202	5	2304	5	10	NULL	0	NULL	statement 2	Process		suggest					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_13_3491_s_184	9642210	(1993) NAD+ binding to the  Escherichia coli K+-uptake protein TrkA and sequence similarity between TrkA and domains of a family of dehydrogenases suggest a role of NAD+ in bacterial transport.	bind
46459	6	2304	5	10	NULL	0	NULL	TrkA	GP	Escherichia coli	is a type of					K+-uptake protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_13_3491_s_184	9642210	(1993) NAD+ binding to the  Escherichia coli K+-uptake protein TrkA and sequence similarity between TrkA and domains of a family of dehydrogenases suggest a role of NAD+ in bacterial transport.	bind
4076	1	2304	6	10	NULL	0	NULL	NAD+	Chemical		bind					TrkA	GP	Escherichia coli			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_13_3491_s_184	9642210	(1993) NAD+ binding to the  Escherichia coli K+-uptake protein TrkA and sequence similarity between TrkA and domains of a family of dehydrogenases suggest a role of NAD+ in bacterial transport.	bind
4077	2	2304	6	10	NULL	0	NULL	TrkA	GP	Escherichia coli	is a type of					K+-uptake protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_13_3491_s_184	9642210	(1993) NAD+ binding to the  Escherichia coli K+-uptake protein TrkA and sequence similarity between TrkA and domains of a family of dehydrogenases suggest a role of NAD+ in bacterial transport.	bind
4078	3	2304	6	10	NULL	0	NULL	NAD+	Chemical		plays a role in					bacterial transport	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_13_3491_s_184	9642210	(1993) NAD+ binding to the  Escherichia coli K+-uptake protein TrkA and sequence similarity between TrkA and domains of a family of dehydrogenases suggest a role of NAD+ in bacterial transport.	bind
46460	4	2304	6	10	NULL	0	NULL	TrkA	GP	sequence	is similar to					dehydrogenases	GP	 family of 	domains of		NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_13_3491_s_184	9642210	(1993) NAD+ binding to the  Escherichia coli K+-uptake protein TrkA and sequence similarity between TrkA and domains of a family of dehydrogenases suggest a role of NAD+ in bacterial transport.	bind
46462	5	2304	6	10	NULL	0	NULL	statement 1	Process		suggest					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_13_3491_s_184	9642210	(1993) NAD+ binding to the  Escherichia coli K+-uptake protein TrkA and sequence similarity between TrkA and domains of a family of dehydrogenases suggest a role of NAD+ in bacterial transport.	bind
46464	6	2304	6	10	NULL	0	NULL	statement 4	Process		suggest					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_13_3491_s_184	9642210	(1993) NAD+ binding to the  Escherichia coli K+-uptake protein TrkA and sequence similarity between TrkA and domains of a family of dehydrogenases suggest a role of NAD+ in bacterial transport.	bind
4203	1	2305	5	10	NULL	0	NULL	NADPH oxidase	GP	phagocyte	bind			Src homology 3 domain		NADPH oxidase	GP	phagocyte	proline-rich targets		NULL		NULL	NULL	NULL	NULL	gw60_embo_21_23_6312_s_366	12456638	(1994) Assembly of the phagocyte NADPH oxidase: binding of Src homology 3 domains to proline-rich targets.	bind
4079	1	2305	6	10	NULL	0	NULL	NADPH oxidase	GP	phagocyte	bind			Src homology 3 domains		NADPH oxidase	GP	phagocyte	proline-rich targets		NULL		NULL	NULL	NULL	NULL	gw60_embo_21_23_6312_s_366	12456638	(1994) Assembly of the phagocyte NADPH oxidase: binding of Src homology 3 domains to proline-rich targets.	bind
4204	1	2306	5	10	NULL	0	NULL	semaphorin	GP		bind									C-SRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39647_s_345	10993894	(1997) A novel transmembrane semaphorin can bind C-SRE  Mol.	bind
46465	2	2306	5	10	NULL	0	NULL	semaphorin	GP		is a type of					transmembrane protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39647_s_345	10993894	(1997) A novel transmembrane semaphorin can bind C-SRE  Mol.	bind
4080	1	2306	6	10	NULL	0	NULL	semaphorin	GP		bind									C-SRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39647_s_345	10993894	(1997) A novel transmembrane semaphorin can bind C-SRE  Mol.	bind
46466	2	2306	6	10	NULL	0	NULL	semaphorin	GP		is a type of					transmembrane protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39647_s_345	10993894	(1997) A novel transmembrane semaphorin can bind C-SRE  Mol.	bind
4205	1	2307	5	10	NULL	0	NULL	kininogen	GP		bind					endothelial cells	Cell	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_3_1521_s_352	10636838	(1997) Binding of high molecular weight kininogen to human endothelial cells is mediated via a site within domains 2 and 3 of the urokinase receptor.	bind
4206	2	2307	5	10	NULL	0	NULL	urokinase receptor	GP		mediate			site with domain 2		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_3_1521_s_352	10636838	(1997) Binding of high molecular weight kininogen to human endothelial cells is mediated via a site within domains 2 and 3 of the urokinase receptor.	bind
5265	3	2307	5	10	NULL	0	NULL	urokinase receptor	GP		mediate			site with domain 3		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_3_1521_s_352	10636838	(1997) Binding of high molecular weight kininogen to human endothelial cells is mediated via a site within domains 2 and 3 of the urokinase receptor.	bind
4081	1	2307	6	10	NULL	0	NULL	kininogen	GP		bind					endothelial cells	Cell	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_3_1521_s_352	10636838	(1997) Binding of high molecular weight kininogen to human endothelial cells is mediated via a site within domains 2 and 3 of the urokinase receptor.	bind
4082	2	2307	6	10	NULL	0	NULL	urokinase receptor	GP		mediates			site within domain 2		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_3_1521_s_352	10636838	(1997) Binding of high molecular weight kininogen to human endothelial cells is mediated via a site within domains 2 and 3 of the urokinase receptor.	bind
4083	3	2307	6	10	NULL	0	NULL	urokinase receptor	GP		mediates			site within domain 3		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_3_1521_s_352	10636838	(1997) Binding of high molecular weight kininogen to human endothelial cells is mediated via a site within domains 2 and 3 of the urokinase receptor.	bind
4207	1	2308	5	10	NULL	0	NULL	FtsZ	GP		bind		directly			ZipA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_13_3486_s_156	9642209	(1997) Direct binding of FtsZ to ZipA, an essential component of the septal ring structure that mediates cell division in  E. coli.	bind
4208	2	2308	5	10	NULL	0	NULL	ZipA	GP		is a component of					septal ring structure	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_13_3486_s_156	9642209	(1997) Direct binding of FtsZ to ZipA, an essential component of the septal ring structure that mediates cell division in  E. coli.	bind
5266	3	2308	5	10	NULL	0	NULL	septal ring structure	GP		mediate					cell division	Process				NULL	E.coli	NULL	NULL	NULL	NULL	gw60_jbacteriol_180_13_3486_s_156	9642209	(1997) Direct binding of FtsZ to ZipA, an essential component of the septal ring structure that mediates cell division in  E. coli.	bind
4084	1	2308	6	10	NULL	0	NULL	FtsZ	GP		bind		directly			ZipA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_13_3486_s_156	9642209	(1997) Direct binding of FtsZ to ZipA, an essential component of the septal ring structure that mediates cell division in  E. coli.	bind
4085	2	2308	6	10	NULL	0	NULL	ZipA	GP		is a component of					septal ring structure	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_13_3486_s_156	9642209	(1997) Direct binding of FtsZ to ZipA, an essential component of the septal ring structure that mediates cell division in  E. coli.	bind
4086	3	2308	6	10	NULL	0	NULL	septal ring structure	GP		mediates					cell division	Process				NULL	E.coli	NULL	NULL	NULL	NULL	gw60_jbacteriol_180_13_3486_s_156	9642209	(1997) Direct binding of FtsZ to ZipA, an essential component of the septal ring structure that mediates cell division in  E. coli.	bind
4209	1	2309	5	10	NULL	0	NULL	fibroblast growth factor	GP	basic	bind					fibrinogen	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_3_1521_s_271	10636838	(1998) Binding of basic fibroblast growth factor to fibrinogen and fibrin.	bind
4210	2	2309	5	10	NULL	0	NULL	fibroblast growth factor	GP	basic	bind					fibrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_3_1521_s_271	10636838	(1998) Binding of basic fibroblast growth factor to fibrinogen and fibrin.	bind
4087	1	2309	6	10	NULL	0	NULL	fibroblast growth factor	GP	basic	bind					fibrinogen	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_3_1521_s_271	10636838	(1998) Binding of basic fibroblast growth factor to fibrinogen and fibrin.	bind
4088	2	2309	6	10	NULL	0	NULL	fibroblast growth factor	GP	basic	bind					fibrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_3_1521_s_271	10636838	(1998) Binding of basic fibroblast growth factor to fibrinogen and fibrin.	bind
4211	1	2310	5	10	NULL	0	NULL	CcpA	GP		bind					xyn	GP	Bacillus subtilis		cre	NULL		NULL	NULL	NULL	NULL	gw60_embo_20_15_3917_s_383	11483495	(1999) Phosphoryl ation of either crh or HPr mediates binding of CcpA to the  Bacillus subtilis xyn cre and catabolite repression of the  xyn operon.	bind
4212	2	2310	5	10	NULL	0	NULL	crh	GP	phosphorylation of	mediate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_15_3917_s_383	11483495	(1999) Phosphoryl ation of either crh or HPr mediates binding of CcpA to the  Bacillus subtilis xyn cre and catabolite repression of the  xyn operon.	bind
4213	3	2310	5	10	NULL	0	NULL	HPr	GP	phosphorylation of	mediate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_15_3917_s_383	11483495	(1999) Phosphoryl ation of either crh or HPr mediates binding of CcpA to the  Bacillus subtilis xyn cre and catabolite repression of the  xyn operon.	bind
4214	4	2310	5	10	NULL	0	NULL	crh	GP	phosphorylation of	mediate					xyn operon	NucleicAcid	catabolite repression of			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_15_3917_s_383	11483495	(1999) Phosphoryl ation of either crh or HPr mediates binding of CcpA to the  Bacillus subtilis xyn cre and catabolite repression of the  xyn operon.	bind
4215	5	2310	5	10	NULL	0	NULL	HPr	GP	phosphorylation of	mediate					xyn operon	NucleicAcid	catabolite repression of			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_15_3917_s_383	11483495	(1999) Phosphoryl ation of either crh or HPr mediates binding of CcpA to the  Bacillus subtilis xyn cre and catabolite repression of the  xyn operon.	bind
5267	6	2310	5	10	NULL	0	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_15_3917_s_383	11483495	(1999) Phosphoryl ation of either crh or HPr mediates binding of CcpA to the  Bacillus subtilis xyn cre and catabolite repression of the  xyn operon.	bind
5268	7	2310	5	10	NULL	0	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_15_3917_s_383	11483495	(1999) Phosphoryl ation of either crh or HPr mediates binding of CcpA to the  Bacillus subtilis xyn cre and catabolite repression of the  xyn operon.	bind
4089	1	2310	6	10	NULL	0	NULL	CcpA	GP		bind					xyn	GP	Bacillus subtilis 		CRE	NULL		NULL	NULL	NULL	NULL	gw60_embo_20_15_3917_s_383	11483495	(1999) Phosphoryl ation of either crh or HPr mediates binding of CcpA to the  Bacillus subtilis xyn cre and catabolite repression of the  xyn operon.	bind
4090	2	2310	6	10	NULL	0	NULL	crh	GP	phosphorylation of	mediates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_15_3917_s_383	11483495	(1999) Phosphoryl ation of either crh or HPr mediates binding of CcpA to the  Bacillus subtilis xyn cre and catabolite repression of the  xyn operon.	bind
4091	3	2310	6	10	NULL	0	NULL	Hpr	GP	phosphorylation of	mediates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_15_3917_s_383	11483495	(1999) Phosphoryl ation of either crh or HPr mediates binding of CcpA to the  Bacillus subtilis xyn cre and catabolite repression of the  xyn operon.	bind
4092	4	2310	6	10	NULL	0	NULL	crh	GP	phosphorylation of	mediates					Xyn operon	NucleicAcid	catabolite repression of			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_15_3917_s_383	11483495	(1999) Phosphoryl ation of either crh or HPr mediates binding of CcpA to the  Bacillus subtilis xyn cre and catabolite repression of the  xyn operon.	bind
4093	5	2310	6	10	NULL	0	NULL	Hpr	GP	phosphorylation of	mediates					Xyn operon	NucleicAcid	catabolite repression of			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_15_3917_s_383	11483495	(1999) Phosphoryl ation of either crh or HPr mediates binding of CcpA to the  Bacillus subtilis xyn cre and catabolite repression of the  xyn operon.	bind
4987	6	2310	6	10	NULL	0	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_15_3917_s_383	11483495	(1999) Phosphoryl ation of either crh or HPr mediates binding of CcpA to the  Bacillus subtilis xyn cre and catabolite repression of the  xyn operon.	bind
4988	7	2310	6	10	NULL	0	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_15_3917_s_383	11483495	(1999) Phosphoryl ation of either crh or HPr mediates binding of CcpA to the  Bacillus subtilis xyn cre and catabolite repression of the  xyn operon.	bind
4216	1	2311	5	10	NULL	0	NULL	actin	GP		bind					profilin	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_86	11294914	(2)   Three reactions contributed to the observed dissociation rate constant,  kobs: dissociation from free actin (Af), actin bound to wild-type profilin (Awt), and actin bound to Y79R profilin (Amu).	bind
4217	2	2311	5	10	NULL	0	NULL	actin	GP		bind					profilin	GP		Y79R		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_86	11294914	(2)   Three reactions contributed to the observed dissociation rate constant,  kobs: dissociation from free actin (Af), actin bound to wild-type profilin (Awt), and actin bound to Y79R profilin (Amu).	bind
4094	1	2311	6	10	NULL	0	NULL	actin	GP		bind					profilin	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_86	11294914	(2)   Three reactions contributed to the observed dissociation rate constant,  kobs: dissociation from free actin (Af), actin bound to wild-type profilin (Awt), and actin bound to Y79R profilin (Amu).	bind
4095	2	2311	6	10	NULL	0	NULL	actin	GP		bind					profilin	GP		Y79R		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_86	11294914	(2)   Three reactions contributed to the observed dissociation rate constant,  kobs: dissociation from free actin (Af), actin bound to wild-type profilin (Awt), and actin bound to Y79R profilin (Amu).	bind
4220	1	2312	5	10	NULL	0	NULL	p53	GP	total cytoplasmic	bind					Parc	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_1_1_s_33	12526785	(2) A large fraction of total cytoplasmic p53 is bound to Parc.	bind
4096	1	2312	6	10	NULL	0	NULL	p53	GP	total cytoplasmic	bind					Parc	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_1_1_s_33	12526785	(2) A large fraction of total cytoplasmic p53 is bound to Parc.	bind
4221	1	2313	5	10	NULL	0	NULL	Mdv1p	GP		bind					Fis1p	GP		TPR-like binding pocket		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_2_291_s_272	16247028	(2) Assembly begins when Mdv1p binds the Fis1p TPR-like binding pocket.	bind
4097	1	2313	6	10	NULL	0	NULL	Mdv1p	GP		bind					Fis1p	GP		TPR-like binding pocket		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_2_291_s_272	16247028	(2) Assembly begins when Mdv1p binds the Fis1p TPR-like binding pocket.	bind
4222	1	2314	5	10	NULL	0	NULL	AP-1	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-leukoc-biol_67_2_10670587_s_6	10670587	(2) At high (50 microM) concentration  it prevents translocation of PKCalpha, and subsequently inhibits ERK1/ERK2  phosphorylation, DNA binding activities of AP-1 and nuclear factor-KB  transcription factors, and the production of both tested cytokines.	bind
46467	2	2314	5	10	NULL	0	NULL	AP-1	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-leukoc-biol_67_2_10670587_s_6	10670587	(2) At high (50 microM) concentration  it prevents translocation of PKCalpha, and subsequently inhibits ERK1/ERK2  phosphorylation, DNA binding activities of AP-1 and nuclear factor-KB  transcription factors, and the production of both tested cytokines.	bind
46468	3	2314	5	10	NULL	0	NULL	nuclear factor-KB 	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-leukoc-biol_67_2_10670587_s_6	10670587	(2) At high (50 microM) concentration  it prevents translocation of PKCalpha, and subsequently inhibits ERK1/ERK2  phosphorylation, DNA binding activities of AP-1 and nuclear factor-KB  transcription factors, and the production of both tested cytokines.	bind
46469	4	2314	5	10	NULL	0	NULL	nuclear factor-KB 	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-leukoc-biol_67_2_10670587_s_6	10670587	(2) At high (50 microM) concentration  it prevents translocation of PKCalpha, and subsequently inhibits ERK1/ERK2  phosphorylation, DNA binding activities of AP-1 and nuclear factor-KB  transcription factors, and the production of both tested cytokines.	bind
4098	1	2314	6	10	NULL	0	NULL	AP-1	GP		bind					DNA	NucleicAcid			site	NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-leukoc-biol_67_2_10670587_s_6	10670587	(2) At high (50 microM) concentration  it prevents translocation of PKCalpha, and subsequently inhibits ERK1/ERK2  phosphorylation, DNA binding activities of AP-1 and nuclear factor-KB  transcription factors, and the production of both tested cytokines.	bind
4099	2	2314	6	10	NULL	0	NULL	nuclear factor-KB	GP		bind					DNA	NucleicAcid			site	NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-leukoc-biol_67_2_10670587_s_6	10670587	(2) At high (50 microM) concentration  it prevents translocation of PKCalpha, and subsequently inhibits ERK1/ERK2  phosphorylation, DNA binding activities of AP-1 and nuclear factor-KB  transcription factors, and the production of both tested cytokines.	bind
46470	3	2314	6	10	NULL	0	NULL	AP-1 	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-leukoc-biol_67_2_10670587_s_6	10670587	(2) At high (50 microM) concentration  it prevents translocation of PKCalpha, and subsequently inhibits ERK1/ERK2  phosphorylation, DNA binding activities of AP-1 and nuclear factor-KB  transcription factors, and the production of both tested cytokines.	bind
46471	4	2314	6	10	NULL	0	NULL	nuclear factor-KB 	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-leukoc-biol_67_2_10670587_s_6	10670587	(2) At high (50 microM) concentration  it prevents translocation of PKCalpha, and subsequently inhibits ERK1/ERK2  phosphorylation, DNA binding activities of AP-1 and nuclear factor-KB  transcription factors, and the production of both tested cytokines.	bind
4223	1	2315	5	10	NULL	0	NULL	InsP3R	GP		bind					PIP2	GP				NULL	lipid rafts	NULL	NULL	NULL	NULL	gw60_neuron_34_2_173_s_34	11970857	(2) Binding between the InsP3R and PIP2 found in lipid rafts can facilitate rapid signaling.	bind
4225	2	2315	5	10	NULL	0	NULL	statement 1	GP		facilitate					rapid signaling	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_34_2_173_s_34	11970857	(2) Binding between the InsP3R and PIP2 found in lipid rafts can facilitate rapid signaling.	bind
4100	1	2315	6	10	NULL	0	NULL	InsP3R	GP		bind					PIP2	GP				NULL	lipid rafts	NULL	NULL	NULL	NULL	gw60_neuron_34_2_173_s_34	11970857	(2) Binding between the InsP3R and PIP2 found in lipid rafts can facilitate rapid signaling.	bind
4101	2	2315	6	10	NULL	0	NULL	statement 1	Process		facilitate					rapid signaling	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_34_2_173_s_34	11970857	(2) Binding between the InsP3R and PIP2 found in lipid rafts can facilitate rapid signaling.	bind
4226	1	2317	5	10	NULL	0	NULL	PSA	GP		bind					phage-displayed peptides	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_zhejiang-da-xue-xue-bao-yi-xue-ban_34_5_16216051_s_6	16216051	(2) Dot blot  was used to analyze the influence of the alpha-Met-D-mannoside on binding  between PSA and phage-displayed peptides.	bind
4102	1	2317	6	10	NULL	0	NULL	PSA	GP		bind					phage-displayed peptides	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_zhejiang-da-xue-xue-bao-yi-xue-ban_34_5_16216051_s_6	16216051	(2) Dot blot  was used to analyze the influence of the alpha-Met-D-mannoside on binding  between PSA and phage-displayed peptides.	bind
4228	1	2318	5	10	NULL	0	NULL	EHD3	GP		bind					Rab11-FIP2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_163_s_338	16251358	(2) EHD3 also binds to Rab11-FIP2  via EH - NPF interactions and may play an additional role in transport of vesicles  carrying Rab11-FIP2 (and possibly Rab11) from the early endosome to the ERC, where  they function in concert with EHD1 to control recycling from the ERC to the PM.	bind
4229	2	2318	5	10	NULL	0	NULL	statement 1	Process		occurs via					EH - NPF 	GP	interactions			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_163_s_338	16251358	(2) EHD3 also binds to Rab11-FIP2  via EH - NPF interactions and may play an additional role in transport of vesicles  carrying Rab11-FIP2 (and possibly Rab11) from the early endosome to the ERC, where  they function in concert with EHD1 to control recycling from the ERC to the PM.	bind
4867	3	2318	5	10	NULL	0	NULL	vesicles	CellComponent		carry					Rab11-FIP2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_163_s_338	16251358	(2) EHD3 also binds to Rab11-FIP2  via EH - NPF interactions and may play an additional role in transport of vesicles  carrying Rab11-FIP2 (and possibly Rab11) from the early endosome to the ERC, where  they function in concert with EHD1 to control recycling from the ERC to the PM.	bind
4868	4	2318	5	10	NULL	0	NULL	vesicles	CellComponent		carry		possibly			Rab11	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_163_s_338	16251358	(2) EHD3 also binds to Rab11-FIP2  via EH - NPF interactions and may play an additional role in transport of vesicles  carrying Rab11-FIP2 (and possibly Rab11) from the early endosome to the ERC, where  they function in concert with EHD1 to control recycling from the ERC to the PM.	bind
4869	6	2318	5	10	NULL	0	NULL	statement 3	Process		transported to					ERC	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_163_s_338	16251358	(2) EHD3 also binds to Rab11-FIP2  via EH - NPF interactions and may play an additional role in transport of vesicles  carrying Rab11-FIP2 (and possibly Rab11) from the early endosome to the ERC, where  they function in concert with EHD1 to control recycling from the ERC to the PM.	bind
4870	7	2318	5	10	NULL	0	NULL	statement 4	Process		transported from					early endosomes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_163_s_338	16251358	(2) EHD3 also binds to Rab11-FIP2  via EH - NPF interactions and may play an additional role in transport of vesicles  carrying Rab11-FIP2 (and possibly Rab11) from the early endosome to the ERC, where  they function in concert with EHD1 to control recycling from the ERC to the PM.	bind
4871	8	2318	5	10	NULL	0	NULL	statement 4	Process		transported to					ERC	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_163_s_338	16251358	(2) EHD3 also binds to Rab11-FIP2  via EH - NPF interactions and may play an additional role in transport of vesicles  carrying Rab11-FIP2 (and possibly Rab11) from the early endosome to the ERC, where  they function in concert with EHD1 to control recycling from the ERC to the PM.	bind
4872	11	2318	5	10	NULL	0	NULL	statement 9	Process		function in					EHD1	GP	 concert with			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_163_s_338	16251358	(2) EHD3 also binds to Rab11-FIP2  via EH - NPF interactions and may play an additional role in transport of vesicles  carrying Rab11-FIP2 (and possibly Rab11) from the early endosome to the ERC, where  they function in concert with EHD1 to control recycling from the ERC to the PM.	bind
52994	5	2318	5	10	NULL	0	NULL	statement 3	Process		transported from					early endosomes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_163_s_338	16251358	(2) EHD3 also binds to Rab11-FIP2  via EH - NPF interactions and may play an additional role in transport of vesicles  carrying Rab11-FIP2 (and possibly Rab11) from the early endosome to the ERC, where  they function in concert with EHD1 to control recycling from the ERC to the PM.	bind
52999	9	2318	5	10	NULL	0	NULL	statement 6	Process		occur after					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_163_s_338	16251358	(2) EHD3 also binds to Rab11-FIP2  via EH - NPF interactions and may play an additional role in transport of vesicles  carrying Rab11-FIP2 (and possibly Rab11) from the early endosome to the ERC, where  they function in concert with EHD1 to control recycling from the ERC to the PM.	bind
53000	10	2318	5	10	NULL	0	NULL	statement 8	Process		occur after					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_163_s_338	16251358	(2) EHD3 also binds to Rab11-FIP2  via EH - NPF interactions and may play an additional role in transport of vesicles  carrying Rab11-FIP2 (and possibly Rab11) from the early endosome to the ERC, where  they function in concert with EHD1 to control recycling from the ERC to the PM.	bind
53001	12	2318	5	10	NULL	0	NULL	statement 10	Process		function in					EHD1	GP	concert with			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_163_s_338	16251358	(2) EHD3 also binds to Rab11-FIP2  via EH - NPF interactions and may play an additional role in transport of vesicles  carrying Rab11-FIP2 (and possibly Rab11) from the early endosome to the ERC, where  they function in concert with EHD1 to control recycling from the ERC to the PM.	bind
4634	1	2318	6	10	NULL	0	NULL	EHD3	GP		bind					Rab11-FIP2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_163_s_338	16251358	(2) EHD3 also binds to Rab11-FIP2  via EH - NPF interactions and may play an additional role in transport of vesicles  carrying Rab11-FIP2 (and possibly Rab11) from the early endosome to the ERC, where  they function in concert with EHD1 to control recycling from the ERC to the PM.	bind
4635	2	2318	6	10	NULL	0	NULL	statement 1	Process		via					EH - NPF interactions	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_163_s_338	16251358	(2) EHD3 also binds to Rab11-FIP2  via EH - NPF interactions and may play an additional role in transport of vesicles  carrying Rab11-FIP2 (and possibly Rab11) from the early endosome to the ERC, where  they function in concert with EHD1 to control recycling from the ERC to the PM.	bind
4636	3	2318	6	10	NULL	0	NULL	vesicles	CellComponent		carry					Rab11-FIP2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_163_s_338	16251358	(2) EHD3 also binds to Rab11-FIP2  via EH - NPF interactions and may play an additional role in transport of vesicles  carrying Rab11-FIP2 (and possibly Rab11) from the early endosome to the ERC, where  they function in concert with EHD1 to control recycling from the ERC to the PM.	bind
4637	4	2318	6	10	NULL	0	NULL	vesicles	CellComponent		carry		possibly			Rab11	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_163_s_338	16251358	(2) EHD3 also binds to Rab11-FIP2  via EH - NPF interactions and may play an additional role in transport of vesicles  carrying Rab11-FIP2 (and possibly Rab11) from the early endosome to the ERC, where  they function in concert with EHD1 to control recycling from the ERC to the PM.	bind
4638	5	2318	6	10	NULL	0	NULL	statement 3	Process		transported from					early endosomes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_163_s_338	16251358	(2) EHD3 also binds to Rab11-FIP2  via EH - NPF interactions and may play an additional role in transport of vesicles  carrying Rab11-FIP2 (and possibly Rab11) from the early endosome to the ERC, where  they function in concert with EHD1 to control recycling from the ERC to the PM.	bind
4639	6	2318	6	10	NULL	0	NULL	statement 3	Process		transported to					ERC	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_163_s_338	16251358	(2) EHD3 also binds to Rab11-FIP2  via EH - NPF interactions and may play an additional role in transport of vesicles  carrying Rab11-FIP2 (and possibly Rab11) from the early endosome to the ERC, where  they function in concert with EHD1 to control recycling from the ERC to the PM.	bind
4640	7	2318	6	10	NULL	0	NULL	statement 4	Process		transported from					early endosomes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_163_s_338	16251358	(2) EHD3 also binds to Rab11-FIP2  via EH - NPF interactions and may play an additional role in transport of vesicles  carrying Rab11-FIP2 (and possibly Rab11) from the early endosome to the ERC, where  they function in concert with EHD1 to control recycling from the ERC to the PM.	bind
53002	8	2318	6	10	NULL	0	NULL	statement 4	Process		transported to					ERC	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_163_s_338	16251358	(2) EHD3 also binds to Rab11-FIP2  via EH - NPF interactions and may play an additional role in transport of vesicles  carrying Rab11-FIP2 (and possibly Rab11) from the early endosome to the ERC, where  they function in concert with EHD1 to control recycling from the ERC to the PM.	bind
53003	9	2318	6	10	NULL	0	NULL	statement 6	Process		occur after					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_163_s_338	16251358	(2) EHD3 also binds to Rab11-FIP2  via EH - NPF interactions and may play an additional role in transport of vesicles  carrying Rab11-FIP2 (and possibly Rab11) from the early endosome to the ERC, where  they function in concert with EHD1 to control recycling from the ERC to the PM.	bind
53004	10	2318	6	10	NULL	0	NULL	statement 8	Process		occur after					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_163_s_338	16251358	(2) EHD3 also binds to Rab11-FIP2  via EH - NPF interactions and may play an additional role in transport of vesicles  carrying Rab11-FIP2 (and possibly Rab11) from the early endosome to the ERC, where  they function in concert with EHD1 to control recycling from the ERC to the PM.	bind
53005	11	2318	6	10	NULL	0	NULL	statement 9	Process		function in					EHD1	GP	concert with			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_163_s_338	16251358	(2) EHD3 also binds to Rab11-FIP2  via EH - NPF interactions and may play an additional role in transport of vesicles  carrying Rab11-FIP2 (and possibly Rab11) from the early endosome to the ERC, where  they function in concert with EHD1 to control recycling from the ERC to the PM.	bind
53006	12	2318	6	10	NULL	0	NULL	statement 10	Process		function in					EHD1	GP	concert with			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_163_s_338	16251358	(2) EHD3 also binds to Rab11-FIP2  via EH - NPF interactions and may play an additional role in transport of vesicles  carrying Rab11-FIP2 (and possibly Rab11) from the early endosome to the ERC, where  they function in concert with EHD1 to control recycling from the ERC to the PM.	bind
4147	1	2319	6	10	NULL	0	NULL	gene regulatory protein	GP	unidentified	bind		hypothetically			RNR3	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_4_502_s_292	12600943	(2) Even if an unidentified gene regulatory protein binds to the  RNR3 promoter, it is insufficient to maintain the presence of SWI/SNF and PIC components at the promoter.	bind
4277	1	2320	5	10	NULL	0	NULL	IQ peptides	GP	free	bind					calmodulin	GP	endogenous			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_22_7_2487_s_252	11923413	(2) High concentrations of free IQ peptides, which should bind to endogenous calmodulin, had no effect on Myo1c binding.	bind
4278	2	2320	5	10	NULL	0	NULL	statement 1	Process		does not effect					Myo1c	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_22_7_2487_s_252	11923413	(2) High concentrations of free IQ peptides, which should bind to endogenous calmodulin, had no effect on Myo1c binding.	bind
4148	1	2320	6	10	NULL	0	NULL	IQ peptides	GP	free	bind					calmodulin	GP	endogenous			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_22_7_2487_s_252	11923413	(2) High concentrations of free IQ peptides, which should bind to endogenous calmodulin, had no effect on Myo1c binding.	bind
4149	2	2320	6	10	NULL	0	NULL	statement 1	Process		has no effect on					Myo1c	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_22_7_2487_s_252	11923413	(2) High concentrations of free IQ peptides, which should bind to endogenous calmodulin, had no effect on Myo1c binding.	bind
4279	1	2321	5	10	NULL	0	NULL	anti-CRP antibody	GP	labeled	bind					FcgammaRIIa receptors	GP				NULL	in antibody solution	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2372_s_172	15486314	(2) In contrast, binding of labeled anti-CRP antibody alone to FcgammaRIIa receptors can only be observed as long as the antibody is present in solution.	bind
4150	1	2321	6	10	NULL	0	NULL	anti-CRP antibody	GP	labeled	bind					FcgammaRIIa receptors	GP				NULL	in antibody solution	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2372_s_172	15486314	(2) In contrast, binding of labeled anti-CRP antibody alone to FcgammaRIIa receptors can only be observed as long as the antibody is present in solution.	bind
4281	1	2322	5	10	NULL	0	NULL	CCR4-NOT protein	GP		bind		directly			TBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_genetics_155_3_1045_s_226	10880468	(2) It is possible that the CCR4-NOT proteins bind directly to TBP and prevent the interaction of TBP with other stabilizing factors like TFIIA and SPT3.	bind
4282	2	2322	5	10	NULL	0	NULL	TBP	GP		interact					TFIIA	GP				NULL		NULL	NULL	NULL	NULL	gw60_genetics_155_3_1045_s_226	10880468	(2) It is possible that the CCR4-NOT proteins bind directly to TBP and prevent the interaction of TBP with other stabilizing factors like TFIIA and SPT3.	bind
4283	3	2322	5	10	NULL	0	NULL	TBP	GP		interact					SPT3	GP				NULL		NULL	NULL	NULL	NULL	gw60_genetics_155_3_1045_s_226	10880468	(2) It is possible that the CCR4-NOT proteins bind directly to TBP and prevent the interaction of TBP with other stabilizing factors like TFIIA and SPT3.	bind
4284	4	2322	5	10	NULL	0	NULL	statement 1	Process		prevent					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_genetics_155_3_1045_s_226	10880468	(2) It is possible that the CCR4-NOT proteins bind directly to TBP and prevent the interaction of TBP with other stabilizing factors like TFIIA and SPT3.	bind
4285	5	2322	5	10	NULL	0	NULL	statement 1	Process		prevent					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_genetics_155_3_1045_s_226	10880468	(2) It is possible that the CCR4-NOT proteins bind directly to TBP and prevent the interaction of TBP with other stabilizing factors like TFIIA and SPT3.	bind
46472	6	2322	5	10	NULL	0	NULL	TFIIA	GP		is a type of					stabilizing factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_genetics_155_3_1045_s_226	10880468	(2) It is possible that the CCR4-NOT proteins bind directly to TBP and prevent the interaction of TBP with other stabilizing factors like TFIIA and SPT3.	bind
46473	7	2322	5	10	NULL	0	NULL	SPT3	GP		is a type of					stabilizing factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_genetics_155_3_1045_s_226	10880468	(2) It is possible that the CCR4-NOT proteins bind directly to TBP and prevent the interaction of TBP with other stabilizing factors like TFIIA and SPT3.	bind
4151	1	2322	6	10	NULL	0	NULL	CCR4-NOT protein	GP		bind		directly			TBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_genetics_155_3_1045_s_226	10880468	(2) It is possible that the CCR4-NOT proteins bind directly to TBP and prevent the interaction of TBP with other stabilizing factors like TFIIA and SPT3.	bind
4152	2	2322	6	10	NULL	0	NULL	TBP	GP		interact with					TFIIA	GP				NULL		NULL	NULL	NULL	NULL	gw60_genetics_155_3_1045_s_226	10880468	(2) It is possible that the CCR4-NOT proteins bind directly to TBP and prevent the interaction of TBP with other stabilizing factors like TFIIA and SPT3.	bind
4153	3	2322	6	10	NULL	0	NULL	TBP	GP		interact with					SPT3	GP				NULL		NULL	NULL	NULL	NULL	gw60_genetics_155_3_1045_s_226	10880468	(2) It is possible that the CCR4-NOT proteins bind directly to TBP and prevent the interaction of TBP with other stabilizing factors like TFIIA and SPT3.	bind
4154	4	2322	6	10	NULL	0	NULL	statement 1	Process		prevents					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_genetics_155_3_1045_s_226	10880468	(2) It is possible that the CCR4-NOT proteins bind directly to TBP and prevent the interaction of TBP with other stabilizing factors like TFIIA and SPT3.	bind
4155	5	2322	6	10	NULL	0	NULL	statement 1	Process		prevents					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_genetics_155_3_1045_s_226	10880468	(2) It is possible that the CCR4-NOT proteins bind directly to TBP and prevent the interaction of TBP with other stabilizing factors like TFIIA and SPT3.	bind
46474	6	2322	6	10	NULL	0	NULL	TFIIA	GP		is a type of					stabilizing factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_genetics_155_3_1045_s_226	10880468	(2) It is possible that the CCR4-NOT proteins bind directly to TBP and prevent the interaction of TBP with other stabilizing factors like TFIIA and SPT3.	bind
46475	7	2322	6	10	NULL	0	NULL	SPT3	GP		is a type of					stabilizing factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_genetics_155_3_1045_s_226	10880468	(2) It is possible that the CCR4-NOT proteins bind directly to TBP and prevent the interaction of TBP with other stabilizing factors like TFIIA and SPT3.	bind
4286	1	2323	5	10	NULL	0	NULL	SRF	GP		bind									CArG B	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_81_4_600_s_253	9314842	(2) MHox enhanced SRF binding to CArG B (Fig 6  ).	bind
4287	2	2323	5	10	NULL	0	NULL	MHox	GP		enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_81_4_600_s_253	9314842	(2) MHox enhanced SRF binding to CArG B (Fig 6  ).	bind
4156	1	2323	6	10	NULL	0	NULL	SRF	GP		bind									CArG B	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_81_4_600_s_253	9314842	(2) MHox enhanced SRF binding to CArG B (Fig 6  ).	bind
4157	2	2323	6	10	NULL	0	NULL	MHox	GP		enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_81_4_600_s_253	9314842	(2) MHox enhanced SRF binding to CArG B (Fig 6  ).	bind
4288	1	2324	5	10	NULL	0	NULL	 CbbR dimer	GP		bind					IR1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_4_1245_s_237	12562794	(2) One CbbR dimer bound to IR1.	bind
4158	1	2324	6	10	NULL	0	NULL	CbbR dimer	GP		bind					IR1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_4_1245_s_237	12562794	(2) One CbbR dimer bound to IR1.	bind
4289	1	2325	5	10	NULL	0	NULL	CSP	GP		bind					Hsc70	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_31_6_987_s_308	11580898	(2) Simultaneous binding of CSP and SGT to Hsc70 maximally stimulates the ATPase activity of Hsc70 to a level 19-fold higherR than that of Hsc70 alone.	bind
4290	2	2325	5	10	NULL	0	NULL	SGT	GP		bind					Hsc70	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_31_6_987_s_308	11580898	(2) Simultaneous binding of CSP and SGT to Hsc70 maximally stimulates the ATPase activity of Hsc70 to a level 19-fold higherR than that of Hsc70 alone.	bind
4291	3	2325	5	10	NULL	0	NULL	statement 1	Process		occurs simultaneously with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_31_6_987_s_308	11580898	(2) Simultaneous binding of CSP and SGT to Hsc70 maximally stimulates the ATPase activity of Hsc70 to a level 19-fold higherR than that of Hsc70 alone.	bind
4292	5	2325	5	10	NULL	0	NULL	statement 3	Process		stimulate					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_31_6_987_s_308	11580898	(2) Simultaneous binding of CSP and SGT to Hsc70 maximally stimulates the ATPase activity of Hsc70 to a level 19-fold higherR than that of Hsc70 alone.	bind
53007	4	2325	5	10	NULL	0	NULL	Hsc70	GP		activates					ATPase	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_31_6_987_s_308	11580898	(2) Simultaneous binding of CSP and SGT to Hsc70 maximally stimulates the ATPase activity of Hsc70 to a level 19-fold higherR than that of Hsc70 alone.	bind
4159	1	2325	6	10	NULL	0	NULL	CSP	GP		bind					Hsc70	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_31_6_987_s_308	11580898	(2) Simultaneous binding of CSP and SGT to Hsc70 maximally stimulates the ATPase activity of Hsc70 to a level 19-fold higherR than that of Hsc70 alone.	bind
4160	2	2325	6	10	NULL	0	NULL	SGT	GP		bind					Hsc70	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_31_6_987_s_308	11580898	(2) Simultaneous binding of CSP and SGT to Hsc70 maximally stimulates the ATPase activity of Hsc70 to a level 19-fold higherR than that of Hsc70 alone.	bind
4161	3	2325	6	10	NULL	0	NULL	statement 1	Process		occurs simultaneously with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_31_6_987_s_308	11580898	(2) Simultaneous binding of CSP and SGT to Hsc70 maximally stimulates the ATPase activity of Hsc70 to a level 19-fold higherR than that of Hsc70 alone.	bind
4162	5	2325	6	10	NULL	0	NULL	statement 3	Process		stimulates					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_31_6_987_s_308	11580898	(2) Simultaneous binding of CSP and SGT to Hsc70 maximally stimulates the ATPase activity of Hsc70 to a level 19-fold higherR than that of Hsc70 alone.	bind
53008	4	2325	6	10	NULL	0	NULL	Hsc70	GP		activates					ATPase	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_31_6_987_s_308	11580898	(2) Simultaneous binding of CSP and SGT to Hsc70 maximally stimulates the ATPase activity of Hsc70 to a level 19-fold higherR than that of Hsc70 alone.	bind
4293	1	2328	5	10	NULL	0	NULL	signal receptor	GP	soluble	bind					cognate membrane receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_4_491_s_43	12600313	(2) The ribosome nascent chain complex (RNC) is targeted to the membrane by the binding of the soluble signal receptor to a cognate membrane receptor.	bind
4294	2	2328	5	10	NULL	0	NULL	RNC	GP		is targeted to					membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_4_491_s_43	12600313	(2) The ribosome nascent chain complex (RNC) is targeted to the membrane by the binding of the soluble signal receptor to a cognate membrane receptor.	bind
4295	3	2328	5	10	NULL	0	NULL	RNC 	GP		is					ribosome nascent chain complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_4_491_s_43	12600313	(2) The ribosome nascent chain complex (RNC) is targeted to the membrane by the binding of the soluble signal receptor to a cognate membrane receptor.	bind
4296	4	2328	5	10	NULL	0	NULL	statement 2	Process		is required for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_4_491_s_43	12600313	(2) The ribosome nascent chain complex (RNC) is targeted to the membrane by the binding of the soluble signal receptor to a cognate membrane receptor.	bind
4163	1	2328	6	10	NULL	0	NULL	signal receptor	GP	soluble	bind					cognate membrane receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_4_491_s_43	12600313	(2) The ribosome nascent chain complex (RNC) is targeted to the membrane by the binding of the soluble signal receptor to a cognate membrane receptor.	bind
4164	2	2328	6	10	NULL	0	NULL	RNC	GP		targeted to					membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_4_491_s_43	12600313	(2) The ribosome nascent chain complex (RNC) is targeted to the membrane by the binding of the soluble signal receptor to a cognate membrane receptor.	bind
4165	3	2328	6	10	NULL	0	NULL	RNC  	GP		is					ribosome nascent chain complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_4_491_s_43	12600313	(2) The ribosome nascent chain complex (RNC) is targeted to the membrane by the binding of the soluble signal receptor to a cognate membrane receptor.	bind
4166	4	2328	6	10	NULL	0	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_4_491_s_43	12600313	(2) The ribosome nascent chain complex (RNC) is targeted to the membrane by the binding of the soluble signal receptor to a cognate membrane receptor.	bind
4357	1	2329	5	10	NULL	0	NULL	AK	GP	one native form of	bind					AMP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_528_1_161_s_40	12297297	(2) There are two native forms of AK existing in solution, of which one binds with substrates AMP, MgATP, as well as ANS and AP5A, whereas the other binds with ADP and MgADP but not with ANS and AP5A.	bind
4358	2	2329	5	10	NULL	0	NULL	AK	GP	one native form of	bind					MgATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_528_1_161_s_40	12297297	(2) There are two native forms of AK existing in solution, of which one binds with substrates AMP, MgATP, as well as ANS and AP5A, whereas the other binds with ADP and MgADP but not with ANS and AP5A.	bind
4359	4	2329	5	10	NULL	0	NULL	AK	GP	one native form of	bind					ANS	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_528_1_161_s_40	12297297	(2) There are two native forms of AK existing in solution, of which one binds with substrates AMP, MgATP, as well as ANS and AP5A, whereas the other binds with ADP and MgADP but not with ANS and AP5A.	bind
4360	3	2329	5	10	NULL	0	NULL	AK	GP	one native form of	bind					AP5A	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_528_1_161_s_40	12297297	(2) There are two native forms of AK existing in solution, of which one binds with substrates AMP, MgATP, as well as ANS and AP5A, whereas the other binds with ADP and MgADP but not with ANS and AP5A.	bind
4361	6	2329	5	10	NULL	0	NULL	AK	GP	other native form of	bind					ADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_528_1_161_s_40	12297297	(2) There are two native forms of AK existing in solution, of which one binds with substrates AMP, MgATP, as well as ANS and AP5A, whereas the other binds with ADP and MgADP but not with ANS and AP5A.	bind
4362	7	2329	5	10	NULL	0	NULL	AK	GP	other native form of	bind					MgADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_528_1_161_s_40	12297297	(2) There are two native forms of AK existing in solution, of which one binds with substrates AMP, MgATP, as well as ANS and AP5A, whereas the other binds with ADP and MgADP but not with ANS and AP5A.	bind
4363	8	2329	5	10	NULL	0	NULL	AK	GP	other native form of	does not bind					ANS	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_528_1_161_s_40	12297297	(2) There are two native forms of AK existing in solution, of which one binds with substrates AMP, MgATP, as well as ANS and AP5A, whereas the other binds with ADP and MgADP but not with ANS and AP5A.	bind
4364	5	2329	5	10	NULL	0	NULL	AK	GP	other native form of	does not bind					AP5A	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_528_1_161_s_40	12297297	(2) There are two native forms of AK existing in solution, of which one binds with substrates AMP, MgATP, as well as ANS and AP5A, whereas the other binds with ADP and MgADP but not with ANS and AP5A.	bind
4167	1	2329	6	10	NULL	0	NULL	AK 	GP	one native form of	bind					AMP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_528_1_161_s_40	12297297	(2) There are two native forms of AK existing in solution, of which one binds with substrates AMP, MgATP, as well as ANS and AP5A, whereas the other binds with ADP and MgADP but not with ANS and AP5A.	bind
4168	2	2329	6	10	NULL	0	NULL	AK	GP	one native form of	bind					MgATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_528_1_161_s_40	12297297	(2) There are two native forms of AK existing in solution, of which one binds with substrates AMP, MgATP, as well as ANS and AP5A, whereas the other binds with ADP and MgADP but not with ANS and AP5A.	bind
4169	3	2329	6	10	NULL	0	NULL	AK 	GP	one native form of	bind					ANS	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_528_1_161_s_40	12297297	(2) There are two native forms of AK existing in solution, of which one binds with substrates AMP, MgATP, as well as ANS and AP5A, whereas the other binds with ADP and MgADP but not with ANS and AP5A.	bind
4170	4	2329	6	10	NULL	0	NULL	AK	GP	one native form of	bind					AP5A	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_528_1_161_s_40	12297297	(2) There are two native forms of AK existing in solution, of which one binds with substrates AMP, MgATP, as well as ANS and AP5A, whereas the other binds with ADP and MgADP but not with ANS and AP5A.	bind
4171	5	2329	6	10	NULL	0	NULL	AK 	GP	other native form of	bind					ADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_528_1_161_s_40	12297297	(2) There are two native forms of AK existing in solution, of which one binds with substrates AMP, MgATP, as well as ANS and AP5A, whereas the other binds with ADP and MgADP but not with ANS and AP5A.	bind
4172	6	2329	6	10	NULL	0	NULL	AK 	GP	other native form of	bind					MgADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_528_1_161_s_40	12297297	(2) There are two native forms of AK existing in solution, of which one binds with substrates AMP, MgATP, as well as ANS and AP5A, whereas the other binds with ADP and MgADP but not with ANS and AP5A.	bind
4173	7	2329	6	10	NULL	0	NULL	AK 	GP	other native form of	does not bind					ANS	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_528_1_161_s_40	12297297	(2) There are two native forms of AK existing in solution, of which one binds with substrates AMP, MgATP, as well as ANS and AP5A, whereas the other binds with ADP and MgADP but not with ANS and AP5A.	bind
4174	8	2329	6	10	NULL	0	NULL	AK 	GP	other native form of	does not bind					AP5A	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_528_1_161_s_40	12297297	(2) There are two native forms of AK existing in solution, of which one binds with substrates AMP, MgATP, as well as ANS and AP5A, whereas the other binds with ADP and MgADP but not with ANS and AP5A.	bind
4369	1	2330	5	10	NULL	0	NULL	cellular membrane	CellComponent		is linked to					actin cytoskeleton	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_133_s_248	11581290	(2) This pili- dependent adhesion induces, through a Rho GTPase-independent pathway, the recruitment of ezrin and moesin, two proteins that link the cellular membrane to the actin cytoskeleton, and the clustering of several transmembrane proteins: ErbB2 and the ezrin binding proteins CD44 and ICAM-1.	bind
4370	2	2330	5	10	NULL	0	NULL	ezrin	GP		is necessary for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_133_s_248	11581290	(2) This pili- dependent adhesion induces, through a Rho GTPase-independent pathway, the recruitment of ezrin and moesin, two proteins that link the cellular membrane to the actin cytoskeleton, and the clustering of several transmembrane proteins: ErbB2 and the ezrin binding proteins CD44 and ICAM-1.	bind
4371	3	2330	5	10	NULL	0	NULL	moesin	GP		is necessary for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_133_s_248	11581290	(2) This pili- dependent adhesion induces, through a Rho GTPase-independent pathway, the recruitment of ezrin and moesin, two proteins that link the cellular membrane to the actin cytoskeleton, and the clustering of several transmembrane proteins: ErbB2 and the ezrin binding proteins CD44 and ICAM-1.	bind
4372	4	2330	5	10	NULL	0	NULL	pili- dependent adhesion	Process		induce					ezrin	GP	recruitment of			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_133_s_248	11581290	(2) This pili- dependent adhesion induces, through a Rho GTPase-independent pathway, the recruitment of ezrin and moesin, two proteins that link the cellular membrane to the actin cytoskeleton, and the clustering of several transmembrane proteins: ErbB2 and the ezrin binding proteins CD44 and ICAM-1.	bind
4373	5	2330	5	10	NULL	0	NULL	statement 4	Process		occurs through					Rho GTPase-independent pathway	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_133_s_248	11581290	(2) This pili- dependent adhesion induces, through a Rho GTPase-independent pathway, the recruitment of ezrin and moesin, two proteins that link the cellular membrane to the actin cytoskeleton, and the clustering of several transmembrane proteins: ErbB2 and the ezrin binding proteins CD44 and ICAM-1.	bind
4374	6	2330	5	10	NULL	0	NULL	pili- dependent adhesion	Process		induce					moesin	GP	recruitment of			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_133_s_248	11581290	(2) This pili- dependent adhesion induces, through a Rho GTPase-independent pathway, the recruitment of ezrin and moesin, two proteins that link the cellular membrane to the actin cytoskeleton, and the clustering of several transmembrane proteins: ErbB2 and the ezrin binding proteins CD44 and ICAM-1.	bind
4375	7	2330	5	10	NULL	0	NULL	statement 6	Process		occurs through					Rho GTPase-independent pathway	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_133_s_248	11581290	(2) This pili- dependent adhesion induces, through a Rho GTPase-independent pathway, the recruitment of ezrin and moesin, two proteins that link the cellular membrane to the actin cytoskeleton, and the clustering of several transmembrane proteins: ErbB2 and the ezrin binding proteins CD44 and ICAM-1.	bind
4376	8	2330	5	10	NULL	0	NULL	CD44	GP		bind					ezrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_133_s_248	11581290	(2) This pili- dependent adhesion induces, through a Rho GTPase-independent pathway, the recruitment of ezrin and moesin, two proteins that link the cellular membrane to the actin cytoskeleton, and the clustering of several transmembrane proteins: ErbB2 and the ezrin binding proteins CD44 and ICAM-1.	bind
4377	9	2330	5	10	NULL	0	NULL	ICAM-1	GP		bind					ezrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_133_s_248	11581290	(2) This pili- dependent adhesion induces, through a Rho GTPase-independent pathway, the recruitment of ezrin and moesin, two proteins that link the cellular membrane to the actin cytoskeleton, and the clustering of several transmembrane proteins: ErbB2 and the ezrin binding proteins CD44 and ICAM-1.	bind
4378	10	2330	5	10	NULL	0	NULL	ErbB2	GP		cluster					statement 8	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_133_s_248	11581290	(2) This pili- dependent adhesion induces, through a Rho GTPase-independent pathway, the recruitment of ezrin and moesin, two proteins that link the cellular membrane to the actin cytoskeleton, and the clustering of several transmembrane proteins: ErbB2 and the ezrin binding proteins CD44 and ICAM-1.	bind
4379	11	2330	5	10	NULL	0	NULL	ErbB2	GP		cluster					statement 9	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_133_s_248	11581290	(2) This pili- dependent adhesion induces, through a Rho GTPase-independent pathway, the recruitment of ezrin and moesin, two proteins that link the cellular membrane to the actin cytoskeleton, and the clustering of several transmembrane proteins: ErbB2 and the ezrin binding proteins CD44 and ICAM-1.	bind
4380	12	2330	5	10	NULL	0	NULL	pili- dependent adhesion	Process		induce					statement 10	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_133_s_248	11581290	(2) This pili- dependent adhesion induces, through a Rho GTPase-independent pathway, the recruitment of ezrin and moesin, two proteins that link the cellular membrane to the actin cytoskeleton, and the clustering of several transmembrane proteins: ErbB2 and the ezrin binding proteins CD44 and ICAM-1.	bind
4381	13	2330	5	10	NULL	0	NULL	pili- dependent adhesion	Process		induce					statement 11	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_133_s_248	11581290	(2) This pili- dependent adhesion induces, through a Rho GTPase-independent pathway, the recruitment of ezrin and moesin, two proteins that link the cellular membrane to the actin cytoskeleton, and the clustering of several transmembrane proteins: ErbB2 and the ezrin binding proteins CD44 and ICAM-1.	bind
4382	14	2330	5	10	NULL	0	NULL	statement 12	Process		occurs through					Rho GTPase-independent pathway	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_133_s_248	11581290	(2) This pili- dependent adhesion induces, through a Rho GTPase-independent pathway, the recruitment of ezrin and moesin, two proteins that link the cellular membrane to the actin cytoskeleton, and the clustering of several transmembrane proteins: ErbB2 and the ezrin binding proteins CD44 and ICAM-1.	bind
4383	15	2330	5	10	NULL	0	NULL	statement 13	Process		occurs through					Rho GTPase-independent pathway	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_133_s_248	11581290	(2) This pili- dependent adhesion induces, through a Rho GTPase-independent pathway, the recruitment of ezrin and moesin, two proteins that link the cellular membrane to the actin cytoskeleton, and the clustering of several transmembrane proteins: ErbB2 and the ezrin binding proteins CD44 and ICAM-1.	bind
4643	1	2330	6	10	NULL	0	NULL	cellular membrane	CellComponent		linked to					actin cytoskeleton	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_133_s_248	11581290	(2) This pili- dependent adhesion induces, through a Rho GTPase-independent pathway, the recruitment of ezrin and moesin, two proteins that link the cellular membrane to the actin cytoskeleton, and the clustering of several transmembrane proteins: ErbB2 and the ezrin binding proteins CD44 and ICAM-1.	bind
4644	4	2330	6	10	NULL	0	NULL	pili- dependent adhesion	Process		induce					ezrin	GP	recruitment of			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_133_s_248	11581290	(2) This pili- dependent adhesion induces, through a Rho GTPase-independent pathway, the recruitment of ezrin and moesin, two proteins that link the cellular membrane to the actin cytoskeleton, and the clustering of several transmembrane proteins: ErbB2 and the ezrin binding proteins CD44 and ICAM-1.	bind
4645	5	2330	6	10	NULL	0	NULL	statement 4	Process		occurs through					Rho GTPase-independent pathway	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_133_s_248	11581290	(2) This pili- dependent adhesion induces, through a Rho GTPase-independent pathway, the recruitment of ezrin and moesin, two proteins that link the cellular membrane to the actin cytoskeleton, and the clustering of several transmembrane proteins: ErbB2 and the ezrin binding proteins CD44 and ICAM-1.	bind
5775	2	2330	6	10	NULL	0	NULL	ezrin	GP		is necessary for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_133_s_248	11581290	(2) This pili- dependent adhesion induces, through a Rho GTPase-independent pathway, the recruitment of ezrin and moesin, two proteins that link the cellular membrane to the actin cytoskeleton, and the clustering of several transmembrane proteins: ErbB2 and the ezrin binding proteins CD44 and ICAM-1.	bind
5776	3	2330	6	10	NULL	0	NULL	moesin	GP		is necessary for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_133_s_248	11581290	(2) This pili- dependent adhesion induces, through a Rho GTPase-independent pathway, the recruitment of ezrin and moesin, two proteins that link the cellular membrane to the actin cytoskeleton, and the clustering of several transmembrane proteins: ErbB2 and the ezrin binding proteins CD44 and ICAM-1.	bind
5777	6	2330	6	10	NULL	0	NULL	pili- dependent adhesion	Process		induce					moesin	GP	recruitment of			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_133_s_248	11581290	(2) This pili- dependent adhesion induces, through a Rho GTPase-independent pathway, the recruitment of ezrin and moesin, two proteins that link the cellular membrane to the actin cytoskeleton, and the clustering of several transmembrane proteins: ErbB2 and the ezrin binding proteins CD44 and ICAM-1.	bind
5778	7	2330	6	10	NULL	0	NULL	statement 6	Process		occurs through					Rho GTPase-independent pathway	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_133_s_248	11581290	(2) This pili- dependent adhesion induces, through a Rho GTPase-independent pathway, the recruitment of ezrin and moesin, two proteins that link the cellular membrane to the actin cytoskeleton, and the clustering of several transmembrane proteins: ErbB2 and the ezrin binding proteins CD44 and ICAM-1.	bind
5779	8	2330	6	10	NULL	0	NULL	CD44	GP		bind					ezrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_133_s_248	11581290	(2) This pili- dependent adhesion induces, through a Rho GTPase-independent pathway, the recruitment of ezrin and moesin, two proteins that link the cellular membrane to the actin cytoskeleton, and the clustering of several transmembrane proteins: ErbB2 and the ezrin binding proteins CD44 and ICAM-1.	bind
5780	9	2330	6	10	NULL	0	NULL	ICAM-1	GP		bind					ezrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_133_s_248	11581290	(2) This pili- dependent adhesion induces, through a Rho GTPase-independent pathway, the recruitment of ezrin and moesin, two proteins that link the cellular membrane to the actin cytoskeleton, and the clustering of several transmembrane proteins: ErbB2 and the ezrin binding proteins CD44 and ICAM-1.	bind
5781	10	2330	6	10	NULL	0	NULL	ErbB2	GP		forms cluster with					statement 8	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_133_s_248	11581290	(2) This pili- dependent adhesion induces, through a Rho GTPase-independent pathway, the recruitment of ezrin and moesin, two proteins that link the cellular membrane to the actin cytoskeleton, and the clustering of several transmembrane proteins: ErbB2 and the ezrin binding proteins CD44 and ICAM-1.	bind
5782	11	2330	6	10	NULL	0	NULL	ErbB2	GP		forms cluster with					statement 9	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_133_s_248	11581290	(2) This pili- dependent adhesion induces, through a Rho GTPase-independent pathway, the recruitment of ezrin and moesin, two proteins that link the cellular membrane to the actin cytoskeleton, and the clustering of several transmembrane proteins: ErbB2 and the ezrin binding proteins CD44 and ICAM-1.	bind
5783	12	2330	6	10	NULL	0	NULL	pili- dependent adhesion	Process		induce					statement 10	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_133_s_248	11581290	(2) This pili- dependent adhesion induces, through a Rho GTPase-independent pathway, the recruitment of ezrin and moesin, two proteins that link the cellular membrane to the actin cytoskeleton, and the clustering of several transmembrane proteins: ErbB2 and the ezrin binding proteins CD44 and ICAM-1.	bind
5784	13	2330	6	10	NULL	0	NULL	pili- dependent adhesion	Process		induce					statement 11	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_133_s_248	11581290	(2) This pili- dependent adhesion induces, through a Rho GTPase-independent pathway, the recruitment of ezrin and moesin, two proteins that link the cellular membrane to the actin cytoskeleton, and the clustering of several transmembrane proteins: ErbB2 and the ezrin binding proteins CD44 and ICAM-1.	bind
5785	14	2330	6	10	NULL	0	NULL	statement 12	Process		occurs through					Rho GTPase-independent pathway	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_133_s_248	11581290	(2) This pili- dependent adhesion induces, through a Rho GTPase-independent pathway, the recruitment of ezrin and moesin, two proteins that link the cellular membrane to the actin cytoskeleton, and the clustering of several transmembrane proteins: ErbB2 and the ezrin binding proteins CD44 and ICAM-1.	bind
5786	15	2330	6	10	NULL	0	NULL	statement 13	Process		occurs through					Rho GTPase-independent pathway	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_133_s_248	11581290	(2) This pili- dependent adhesion induces, through a Rho GTPase-independent pathway, the recruitment of ezrin and moesin, two proteins that link the cellular membrane to the actin cytoskeleton, and the clustering of several transmembrane proteins: ErbB2 and the ezrin binding proteins CD44 and ICAM-1.	bind
4365	1	2331	5	10	NULL	0	NULL	VAF	GP		bind					IRF7	GP			ISRE	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_13_12262_s_214	15664995	(2) VAF upon virus infection also binds to IRF7 ISRE and IRFE and activates IRF7 transcription.	bind
4366	2	2331	5	10	NULL	0	NULL	VAF	GP		bind					IRF7	GP			IRFE	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_13_12262_s_214	15664995	(2) VAF upon virus infection also binds to IRF7 ISRE and IRFE and activates IRF7 transcription.	bind
4367	3	2331	5	10	NULL	0	NULL	statement 1	Process		activate					IRF7 	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_13_12262_s_214	15664995	(2) VAF upon virus infection also binds to IRF7 ISRE and IRFE and activates IRF7 transcription.	bind
4368	4	2331	5	10	NULL	0	NULL	statement 2	Process		activate					IRF7 	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_13_12262_s_214	15664995	(2) VAF upon virus infection also binds to IRF7 ISRE and IRFE and activates IRF7 transcription.	bind
53013	5	2331	5	10	NULL	0	NULL	statement 1	Process		occur upon					virus	Organism	infection of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_13_12262_s_214	15664995	(2) VAF upon virus infection also binds to IRF7 ISRE and IRFE and activates IRF7 transcription.	bind
53014	6	2331	5	10	NULL	0	NULL	statement 2	Process		occur upon					virus	Organism	infection of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_13_12262_s_214	15664995	(2) VAF upon virus infection also binds to IRF7 ISRE and IRFE and activates IRF7 transcription.	bind
53015	7	2331	5	10	NULL	0	NULL	statement 3	Process		occur upon					virus	Organism	infection of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_13_12262_s_214	15664995	(2) VAF upon virus infection also binds to IRF7 ISRE and IRFE and activates IRF7 transcription.	bind
53016	8	2331	5	10	NULL	0	NULL	statement 4	Process		occur upon					virus	Organism	infection of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_13_12262_s_214	15664995	(2) VAF upon virus infection also binds to IRF7 ISRE and IRFE and activates IRF7 transcription.	bind
4414	1	2331	6	10	NULL	0	NULL	VAF	GP		bind					IRF7	GP			ISRE	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_13_12262_s_214	15664995	(2) VAF upon virus infection also binds to IRF7 ISRE and IRFE and activates IRF7 transcription.	bind
4416	2	2331	6	10	NULL	0	NULL	statement 1	Process		occurs upon					virus	Organism	infection of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_13_12262_s_214	15664995	(2) VAF upon virus infection also binds to IRF7 ISRE and IRFE and activates IRF7 transcription.	bind
4417	3	2331	6	10	NULL	0	NULL	VAF	GP		bind					IRF7	GP			IRFE	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_13_12262_s_214	15664995	(2) VAF upon virus infection also binds to IRF7 ISRE and IRFE and activates IRF7 transcription.	bind
4418	4	2331	6	10	NULL	0	NULL	statement 3	Process		occurs upon					virus	Organism	infection of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_13_12262_s_214	15664995	(2) VAF upon virus infection also binds to IRF7 ISRE and IRFE and activates IRF7 transcription.	bind
4420	5	2331	6	10	NULL	0	NULL	VAF	GP		activates					IRF7	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_13_12262_s_214	15664995	(2) VAF upon virus infection also binds to IRF7 ISRE and IRFE and activates IRF7 transcription.	bind
4422	6	2331	6	10	NULL	0	NULL	statement 5	Process		occurs upon					virus	Organism	infection of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_13_12262_s_214	15664995	(2) VAF upon virus infection also binds to IRF7 ISRE and IRFE and activates IRF7 transcription.	bind
4384	1	2332	5	10	NULL	0	NULL	ATP	Chemical		bind					KinI	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1422_s_250	15029249	(2) When  ATP binds to KinI, it induces a conformational change in the catalytic core that  pulls the tubulins at the L2 and 'neck'' attachments and pushes in at the  intradimer interface, curving the dimer.	bind
4385	2	2332	5	10	NULL	0	NULL	statement 1	Process		induce							conformational change of	catalytic core		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1422_s_250	15029249	(2) When  ATP binds to KinI, it induces a conformational change in the catalytic core that  pulls the tubulins at the L2 and 'neck'' attachments and pushes in at the  intradimer interface, curving the dimer.	bind
4425	1	2332	6	10	NULL	0	NULL	ATP	Chemical		bind					KinI	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1422_s_250	15029249	(2) When  ATP binds to KinI, it induces a conformational change in the catalytic core that  pulls the tubulins at the L2 and 'neck'' attachments and pushes in at the  intradimer interface, curving the dimer.	bind
4647	2	2332	6	10	NULL	0	NULL	statement 1	Process		induces							conformational change of	catalytic core		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1422_s_250	15029249	(2) When  ATP binds to KinI, it induces a conformational change in the catalytic core that  pulls the tubulins at the L2 and 'neck'' attachments and pushes in at the  intradimer interface, curving the dimer.	bind
4390	1	2333	5	10	NULL	0	NULL	Thiamine derivatives	Chemical		bind		directly			messenger RNAs	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_13_10859_s_824	12556463	(2002) Thiamine derivatives bind messenger RNAs directly to regulate bacterial gene expression.	bind
4391	2	2333	5	10	NULL	0	NULL	statement 1	Process		regulate					gene expression	Process	bacterial			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_13_10859_s_824	12556463	(2002) Thiamine derivatives bind messenger RNAs directly to regulate bacterial gene expression.	bind
53018	3	2333	5	10	NULL	0	NULL	statement 1	Process		lead to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_13_10859_s_824	12556463	(2002) Thiamine derivatives bind messenger RNAs directly to regulate bacterial gene expression.	bind
4524	1	2333	6	10	NULL	0	NULL	Thiamine derivatives	Chemical		bind		directly			mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_13_10859_s_824	12556463	(2002) Thiamine derivatives bind messenger RNAs directly to regulate bacterial gene expression.	bind
4525	2	2333	6	10	NULL	0	NULL	Thiamine derivatives	Chemical		regulates					gene expression	Process	bacterial 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_13_10859_s_824	12556463	(2002) Thiamine derivatives bind messenger RNAs directly to regulate bacterial gene expression.	bind
4526	3	2333	6	10	NULL	0	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_13_10859_s_824	12556463	(2002) Thiamine derivatives bind messenger RNAs directly to regulate bacterial gene expression.	bind
4392	1	2335	5	10	NULL	0	NULL	epsilonATP	Chemical		dissociate from					free actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_87	11294914	(3)   where  kf,  kwt, and  kmu are rate constants for epsilonATP dissociation from free actin, actin bound to wild-type profilin and actin bound to Y79R.	bind
4393	2	2335	5	10	NULL	0	NULL	actin	GP		bind					profilin	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_87	11294914	(3)   where  kf,  kwt, and  kmu are rate constants for epsilonATP dissociation from free actin, actin bound to wild-type profilin and actin bound to Y79R.	bind
4394	3	2335	5	10	NULL	0	NULL	epsilonATP	Chemical		dissociate from					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_87	11294914	(3)   where  kf,  kwt, and  kmu are rate constants for epsilonATP dissociation from free actin, actin bound to wild-type profilin and actin bound to Y79R.	bind
4395	4	2335	5	10	NULL	0	NULL	actin	GP		bind								Y79R		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_87	11294914	(3)   where  kf,  kwt, and  kmu are rate constants for epsilonATP dissociation from free actin, actin bound to wild-type profilin and actin bound to Y79R.	bind
4396	5	2335	5	10	NULL	0	NULL	epsilonATP	Chemical		dissociate from					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_87	11294914	(3)   where  kf,  kwt, and  kmu are rate constants for epsilonATP dissociation from free actin, actin bound to wild-type profilin and actin bound to Y79R.	bind
4527	1	2335	6	10	NULL	0	NULL	actin	GP		bind					profilin	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_87	11294914	(3)   where  kf,  kwt, and  kmu are rate constants for epsilonATP dissociation from free actin, actin bound to wild-type profilin and actin bound to Y79R.	bind
4528	2	2335	6	10	NULL	0	NULL	actin	GP		bind								Y79R		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_87	11294914	(3)   where  kf,  kwt, and  kmu are rate constants for epsilonATP dissociation from free actin, actin bound to wild-type profilin and actin bound to Y79R.	bind
53020	3	2335	6	10	NULL	0	NULL	epsilonATP	Chemical		dissociate from					free actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_87	11294914	(3)   where  kf,  kwt, and  kmu are rate constants for epsilonATP dissociation from free actin, actin bound to wild-type profilin and actin bound to Y79R.	bind
53021	5	2335	6	10	NULL	0	NULL	epsilonATP	Chemical		dissociate from					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_87	11294914	(3)   where  kf,  kwt, and  kmu are rate constants for epsilonATP dissociation from free actin, actin bound to wild-type profilin and actin bound to Y79R.	bind
53025	4	2335	6	10	NULL	0	NULL	epsilonATP	Chemical		dissociate from					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_87	11294914	(3)   where  kf,  kwt, and  kmu are rate constants for epsilonATP dissociation from free actin, actin bound to wild-type profilin and actin bound to Y79R.	bind
4400	1	2336	5	10	NULL	0	NULL	CcpA	GP		bind		specifically			gnt gene	GP	B. subtilis		CRE	NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_19_3_187_s_129	9050218	(3)  Using gel-retardation analysis, it was demonstrated that specific binding of CcpA  to CRE of the  B. subtilis gnt gene is triggered by HPr(Ser-P) but not by free HPr.	bind
4402	2	2336	5	10	NULL	0	NULL	statement 1	Process		is triggered by					HPr	GP		Ser-P		NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_19_3_187_s_129	9050218	(3)  Using gel-retardation analysis, it was demonstrated that specific binding of CcpA  to CRE of the  B. subtilis gnt gene is triggered by HPr(Ser-P) but not by free HPr.	bind
4403	3	2336	5	10	NULL	0	NULL	statement 1	Process		is not triggered by					HPr	GP	free			NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_19_3_187_s_129	9050218	(3)  Using gel-retardation analysis, it was demonstrated that specific binding of CcpA  to CRE of the  B. subtilis gnt gene is triggered by HPr(Ser-P) but not by free HPr.	bind
4529	1	2336	6	10	NULL	0	NULL	CcpA	GP		bind		specifically			gnt gene	GP	B. subtilis		CRE	NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_19_3_187_s_129	9050218	(3)  Using gel-retardation analysis, it was demonstrated that specific binding of CcpA  to CRE of the  B. subtilis gnt gene is triggered by HPr(Ser-P) but not by free HPr.	bind
4530	2	2336	6	10	NULL	0	NULL	Hpr	GP		triggers			Ser-P		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_19_3_187_s_129	9050218	(3)  Using gel-retardation analysis, it was demonstrated that specific binding of CcpA  to CRE of the  B. subtilis gnt gene is triggered by HPr(Ser-P) but not by free HPr.	bind
4531	3	2336	6	10	NULL	0	NULL	Hpr	GP	free	does not trigger					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_19_3_187_s_129	9050218	(3)  Using gel-retardation analysis, it was demonstrated that specific binding of CcpA  to CRE of the  B. subtilis gnt gene is triggered by HPr(Ser-P) but not by free HPr.	bind
4405	1	2337	5	10	NULL	0	NULL	Apo A-1	GP		bind		possibly;;directly			caveola	GP		FC-rich ;;exofacial face of 		NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1529_1_210_s_171	11111090	(3) Apo A-1 (or pre- -HDL) could bind directly to the FC-rich exofacial face of the caveola to facilitate FC desorption [  93].	bind
4406	2	2337	5	10	NULL	0	NULL	pre- -HDL	Chemical		bind		possibly;;directly			caveola	GP		FC-rich;;exofacial face of		NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1529_1_210_s_171	11111090	(3) Apo A-1 (or pre- -HDL) could bind directly to the FC-rich exofacial face of the caveola to facilitate FC desorption [  93].	bind
4407	3	2337	5	10	NULL	0	NULL	statement 1	Process		facilitate					FC desorption	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1529_1_210_s_171	11111090	(3) Apo A-1 (or pre- -HDL) could bind directly to the FC-rich exofacial face of the caveola to facilitate FC desorption [  93].	bind
4408	4	2337	5	10	NULL	0	NULL	statement 2	Process		facilitate					FC desorption	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1529_1_210_s_171	11111090	(3) Apo A-1 (or pre- -HDL) could bind directly to the FC-rich exofacial face of the caveola to facilitate FC desorption [  93].	bind
5931	5	2337	5	10	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1529_1_210_s_171	11111090	(3) Apo A-1 (or pre- -HDL) could bind directly to the FC-rich exofacial face of the caveola to facilitate FC desorption [  93].	bind
4532	1	2337	6	10	NULL	0	NULL	Apo A-1	GP		bind		possibly ;;directly			 caveola	GP		FC-rich;; exofacial face of		NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1529_1_210_s_171	11111090	(3) Apo A-1 (or pre- -HDL) could bind directly to the FC-rich exofacial face of the caveola to facilitate FC desorption [  93].	bind
4533	2	2337	6	10	NULL	0	NULL	pre- -HDL	Chemical		bind		possibly;;directly			caveola	GP		FC-rich;; exofacial face of		NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1529_1_210_s_171	11111090	(3) Apo A-1 (or pre- -HDL) could bind directly to the FC-rich exofacial face of the caveola to facilitate FC desorption [  93].	bind
4534	3	2337	6	10	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1529_1_210_s_171	11111090	(3) Apo A-1 (or pre- -HDL) could bind directly to the FC-rich exofacial face of the caveola to facilitate FC desorption [  93].	bind
4535	4	2337	6	10	NULL	0	NULL	Apo A-1	GP		facilitate					FC desorption	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1529_1_210_s_171	11111090	(3) Apo A-1 (or pre- -HDL) could bind directly to the FC-rich exofacial face of the caveola to facilitate FC desorption [  93].	bind
4536	5	2337	6	10	NULL	0	NULL	statement 1	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1529_1_210_s_171	11111090	(3) Apo A-1 (or pre- -HDL) could bind directly to the FC-rich exofacial face of the caveola to facilitate FC desorption [  93].	bind
4875	1	2338	5	10	NULL	0	NULL	bicarbonate	Chemical		increase					Mn2+ 	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1503_1_187_s_154	11115633	(3) Bicarbonate increases the Mn2+ binding [ 15], the formation of the Mn cluster capable of water oxidation [ 18 and  22] and stabilizes the WOC [ 19] indirectly, through its binding to other PSII components that is important for structural/functional organization of the whole PSII complex and, in particular, for functional binding of Mn. Govindjee and co-workers [  40] suggested that bicarbonate bound to the acceptor side is required for PSII activity both on the acceptor and the donor sides.	bind
4876	3	2338	5	10	NULL	0	NULL	Mn cluster	Chemical		is capable of					water oxidation	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1503_1_187_s_154	11115633	(3) Bicarbonate increases the Mn2+ binding [ 15], the formation of the Mn cluster capable of water oxidation [ 18 and  22] and stabilizes the WOC [ 19] indirectly, through its binding to other PSII components that is important for structural/functional organization of the whole PSII complex and, in particular, for functional binding of Mn. Govindjee and co-workers [  40] suggested that bicarbonate bound to the acceptor side is required for PSII activity both on the acceptor and the donor sides.	bind
4877	4	2338	5	10	NULL	0	NULL	bicarbonate	Chemical		stabilize		indirectly			WOC	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1503_1_187_s_154	11115633	(3) Bicarbonate increases the Mn2+ binding [ 15], the formation of the Mn cluster capable of water oxidation [ 18 and  22] and stabilizes the WOC [ 19] indirectly, through its binding to other PSII components that is important for structural/functional organization of the whole PSII complex and, in particular, for functional binding of Mn. Govindjee and co-workers [  40] suggested that bicarbonate bound to the acceptor side is required for PSII activity both on the acceptor and the donor sides.	bind
5556	2	2338	5	10	NULL	0	NULL	bicarbonate	Chemical		increase					Mn cluster	Chemical	formation of 			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1503_1_187_s_154	11115633	(3) Bicarbonate increases the Mn2+ binding [ 15], the formation of the Mn cluster capable of water oxidation [ 18 and  22] and stabilizes the WOC [ 19] indirectly, through its binding to other PSII components that is important for structural/functional organization of the whole PSII complex and, in particular, for functional binding of Mn. Govindjee and co-workers [  40] suggested that bicarbonate bound to the acceptor side is required for PSII activity both on the acceptor and the donor sides.	bind
5557	5	2338	5	10	NULL	0	NULL	Bicarbonate	Chemical		bind					PSII components	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1503_1_187_s_154	11115633	(3) Bicarbonate increases the Mn2+ binding [ 15], the formation of the Mn cluster capable of water oxidation [ 18 and  22] and stabilizes the WOC [ 19] indirectly, through its binding to other PSII components that is important for structural/functional organization of the whole PSII complex and, in particular, for functional binding of Mn. Govindjee and co-workers [  40] suggested that bicarbonate bound to the acceptor side is required for PSII activity both on the acceptor and the donor sides.	bind
5558	6	2338	5	10	NULL	0	NULL	statement 5	Process		is required for					whole PSII complex	GP	structural/functional organization of			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1503_1_187_s_154	11115633	(3) Bicarbonate increases the Mn2+ binding [ 15], the formation of the Mn cluster capable of water oxidation [ 18 and  22] and stabilizes the WOC [ 19] indirectly, through its binding to other PSII components that is important for structural/functional organization of the whole PSII complex and, in particular, for functional binding of Mn. Govindjee and co-workers [  40] suggested that bicarbonate bound to the acceptor side is required for PSII activity both on the acceptor and the donor sides.	bind
5559	7	2338	5	10	NULL	0	NULL	statement 5	Process		is required for					Mn	Chemical	functional binding of 			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1503_1_187_s_154	11115633	(3) Bicarbonate increases the Mn2+ binding [ 15], the formation of the Mn cluster capable of water oxidation [ 18 and  22] and stabilizes the WOC [ 19] indirectly, through its binding to other PSII components that is important for structural/functional organization of the whole PSII complex and, in particular, for functional binding of Mn. Govindjee and co-workers [  40] suggested that bicarbonate bound to the acceptor side is required for PSII activity both on the acceptor and the donor sides.	bind
5560	8	2338	5	10	NULL	0	NULL	bicarbonate	Chemical		bind					acceptor side	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1503_1_187_s_154	11115633	(3) Bicarbonate increases the Mn2+ binding [ 15], the formation of the Mn cluster capable of water oxidation [ 18 and  22] and stabilizes the WOC [ 19] indirectly, through its binding to other PSII components that is important for structural/functional organization of the whole PSII complex and, in particular, for functional binding of Mn. Govindjee and co-workers [  40] suggested that bicarbonate bound to the acceptor side is required for PSII activity both on the acceptor and the donor sides.	bind
5561	9	2338	5	10	NULL	0	NULL	statement 8	Process		is required for					PSII	GP	activity of donor sides			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1503_1_187_s_154	11115633	(3) Bicarbonate increases the Mn2+ binding [ 15], the formation of the Mn cluster capable of water oxidation [ 18 and  22] and stabilizes the WOC [ 19] indirectly, through its binding to other PSII components that is important for structural/functional organization of the whole PSII complex and, in particular, for functional binding of Mn. Govindjee and co-workers [  40] suggested that bicarbonate bound to the acceptor side is required for PSII activity both on the acceptor and the donor sides.	bind
5930	10	2338	5	10	NULL	0	NULL	statement 8	Process		is required for					PS II	GP	activity of acceptor sides			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1503_1_187_s_154	11115633	(3) Bicarbonate increases the Mn2+ binding [ 15], the formation of the Mn cluster capable of water oxidation [ 18 and  22] and stabilizes the WOC [ 19] indirectly, through its binding to other PSII components that is important for structural/functional organization of the whole PSII complex and, in particular, for functional binding of Mn. Govindjee and co-workers [  40] suggested that bicarbonate bound to the acceptor side is required for PSII activity both on the acceptor and the donor sides.	bind
53031	11	2338	5	10	NULL	0	NULL	statement 4	Process		occur through					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1503_1_187_s_154	11115633	(3) Bicarbonate increases the Mn2+ binding [ 15], the formation of the Mn cluster capable of water oxidation [ 18 and  22] and stabilizes the WOC [ 19] indirectly, through its binding to other PSII components that is important for structural/functional organization of the whole PSII complex and, in particular, for functional binding of Mn. Govindjee and co-workers [  40] suggested that bicarbonate bound to the acceptor side is required for PSII activity both on the acceptor and the donor sides.	bind
4648	1	2338	6	10	NULL	0	NULL	Bicarbonate	Chemical		increases					Mn+2	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1503_1_187_s_154	11115633	(3) Bicarbonate increases the Mn2+ binding [ 15], the formation of the Mn cluster capable of water oxidation [ 18 and  22] and stabilizes the WOC [ 19] indirectly, through its binding to other PSII components that is important for structural/functional organization of the whole PSII complex and, in particular, for functional binding of Mn. Govindjee and co-workers [  40] suggested that bicarbonate bound to the acceptor side is required for PSII activity both on the acceptor and the donor sides.	bind
4649	2	2338	6	10	NULL	0	NULL	Mn cluster	Chemical		oxidizes					water	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1503_1_187_s_154	11115633	(3) Bicarbonate increases the Mn2+ binding [ 15], the formation of the Mn cluster capable of water oxidation [ 18 and  22] and stabilizes the WOC [ 19] indirectly, through its binding to other PSII components that is important for structural/functional organization of the whole PSII complex and, in particular, for functional binding of Mn. Govindjee and co-workers [  40] suggested that bicarbonate bound to the acceptor side is required for PSII activity both on the acceptor and the donor sides.	bind
4650	3	2338	6	10	NULL	0	NULL	Bicarbonate	Chemical		increases					Mn cluster	Chemical	formation of			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1503_1_187_s_154	11115633	(3) Bicarbonate increases the Mn2+ binding [ 15], the formation of the Mn cluster capable of water oxidation [ 18 and  22] and stabilizes the WOC [ 19] indirectly, through its binding to other PSII components that is important for structural/functional organization of the whole PSII complex and, in particular, for functional binding of Mn. Govindjee and co-workers [  40] suggested that bicarbonate bound to the acceptor side is required for PSII activity both on the acceptor and the donor sides.	bind
4651	4	2338	6	10	NULL	0	NULL	Bicarbonate	Chemical		stabilizes		indirectly			WOC	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1503_1_187_s_154	11115633	(3) Bicarbonate increases the Mn2+ binding [ 15], the formation of the Mn cluster capable of water oxidation [ 18 and  22] and stabilizes the WOC [ 19] indirectly, through its binding to other PSII components that is important for structural/functional organization of the whole PSII complex and, in particular, for functional binding of Mn. Govindjee and co-workers [  40] suggested that bicarbonate bound to the acceptor side is required for PSII activity both on the acceptor and the donor sides.	bind
4652	5	2338	6	10	NULL	0	NULL	Bicarbonate	Chemical		bind					PSII components	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1503_1_187_s_154	11115633	(3) Bicarbonate increases the Mn2+ binding [ 15], the formation of the Mn cluster capable of water oxidation [ 18 and  22] and stabilizes the WOC [ 19] indirectly, through its binding to other PSII components that is important for structural/functional organization of the whole PSII complex and, in particular, for functional binding of Mn. Govindjee and co-workers [  40] suggested that bicarbonate bound to the acceptor side is required for PSII activity both on the acceptor and the donor sides.	bind
4653	6	2338	6	NULL	NULL	0	NULL	Bicarbonate	NULL		bind	NULL					NULL		acceptor side		NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1503_1_187_s_154	11115633	(3) Bicarbonate increases the Mn2+ binding [ 15], the formation of the Mn cluster capable of water oxidation [ 18 and  22] and stabilizes the WOC [ 19] indirectly, through its binding to other PSII components that is important for structural/functional organization of the whole PSII complex and, in particular, for functional binding of Mn. Govindjee and co-workers [  40] suggested that bicarbonate bound to the acceptor side is required for PSII activity both on the acceptor and the donor sides.	bind
4654	7	2338	6	NULL	NULL	0	NULL	statement 6	NULL		is required for	NULL				PSII 	NULL	activity of 	acceptor side		NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1503_1_187_s_154	11115633	(3) Bicarbonate increases the Mn2+ binding [ 15], the formation of the Mn cluster capable of water oxidation [ 18 and  22] and stabilizes the WOC [ 19] indirectly, through its binding to other PSII components that is important for structural/functional organization of the whole PSII complex and, in particular, for functional binding of Mn. Govindjee and co-workers [  40] suggested that bicarbonate bound to the acceptor side is required for PSII activity both on the acceptor and the donor sides.	bind
5743	8	2338	6	NULL	NULL	0	NULL	statement 6	NULL		is required for	NULL				PS II	NULL	activity of	donor side		NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1503_1_187_s_154	11115633	(3) Bicarbonate increases the Mn2+ binding [ 15], the formation of the Mn cluster capable of water oxidation [ 18 and  22] and stabilizes the WOC [ 19] indirectly, through its binding to other PSII components that is important for structural/functional organization of the whole PSII complex and, in particular, for functional binding of Mn. Govindjee and co-workers [  40] suggested that bicarbonate bound to the acceptor side is required for PSII activity both on the acceptor and the donor sides.	bind
53032	9	2338	6	10	NULL	0	NULL	statement 4	NULL		occur through	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1503_1_187_s_154	11115633	(3) Bicarbonate increases the Mn2+ binding [ 15], the formation of the Mn cluster capable of water oxidation [ 18 and  22] and stabilizes the WOC [ 19] indirectly, through its binding to other PSII components that is important for structural/functional organization of the whole PSII complex and, in particular, for functional binding of Mn. Govindjee and co-workers [  40] suggested that bicarbonate bound to the acceptor side is required for PSII activity both on the acceptor and the donor sides.	bind
53033	10	2338	6	10	NULL	0	NULL	statement 5	NULL		is required for	NULL				 whole PSII complex	NULL	structural/functional organization of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1503_1_187_s_154	11115633	(3) Bicarbonate increases the Mn2+ binding [ 15], the formation of the Mn cluster capable of water oxidation [ 18 and  22] and stabilizes the WOC [ 19] indirectly, through its binding to other PSII components that is important for structural/functional organization of the whole PSII complex and, in particular, for functional binding of Mn. Govindjee and co-workers [  40] suggested that bicarbonate bound to the acceptor side is required for PSII activity both on the acceptor and the donor sides.	bind
53034	11	2338	6	10	NULL	0	NULL	statement 5	NULL		is required for	NULL				Mn	NULL	functional binding of 			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1503_1_187_s_154	11115633	(3) Bicarbonate increases the Mn2+ binding [ 15], the formation of the Mn cluster capable of water oxidation [ 18 and  22] and stabilizes the WOC [ 19] indirectly, through its binding to other PSII components that is important for structural/functional organization of the whole PSII complex and, in particular, for functional binding of Mn. Govindjee and co-workers [  40] suggested that bicarbonate bound to the acceptor side is required for PSII activity both on the acceptor and the donor sides.	bind
4409	1	2339	5	10	NULL	0	NULL	GR	GP		bind					glucocorticoid	GP			responsive elements	NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_126_3_537_s_181	10188959	(3) Binding of GR to glucocorticoid responsive elements modulates TF-induced transactivation.	bind
4410	2	2339	5	10	NULL	0	NULL	TF	GP		induce					transactivation	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_126_3_537_s_181	10188959	(3) Binding of GR to glucocorticoid responsive elements modulates TF-induced transactivation.	bind
46477	3	2339	5	10	NULL	0	NULL	statement 1	Process		modulate					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_126_3_537_s_181	10188959	(3) Binding of GR to glucocorticoid responsive elements modulates TF-induced transactivation.	bind
4537	1	2339	6	10	NULL	0	NULL	GR	GP		bind					glucocorticoid	GP			 responsive element	NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_126_3_537_s_181	10188959	(3) Binding of GR to glucocorticoid responsive elements modulates TF-induced transactivation.	bind
4538	2	2339	6	10	NULL	0	NULL	TF	GP		induce					transactivation	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_126_3_537_s_181	10188959	(3) Binding of GR to glucocorticoid responsive elements modulates TF-induced transactivation.	bind
46478	3	2339	6	10	NULL	0	NULL	statement 1	Process		modulate					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_126_3_537_s_181	10188959	(3) Binding of GR to glucocorticoid responsive elements modulates TF-induced transactivation.	bind
4411	1	2340	5	10	NULL	0	NULL	VLA-4	Cell		bind					VCAM-1	GP	endothelial			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_353_s_130	10669630	(3) Binding of monocyte VLA-4 by endothelial VCAM-1 is needed for the induction of IL-1beta in monocytes.	bind
4412	2	2340	5	10	NULL	0	NULL	statement 1	Process		induce					IL-1beta	GP				NULL	monocytes	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_353_s_130	10669630	(3) Binding of monocyte VLA-4 by endothelial VCAM-1 is needed for the induction of IL-1beta in monocytes.	bind
53035	3	2340	5	10	NULL	0	NULL	VLA-4	Cell		is a type of					monocyte	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_353_s_130	10669630	(3) Binding of monocyte VLA-4 by endothelial VCAM-1 is needed for the induction of IL-1beta in monocytes.	bind
4539	1	2340	6	10	NULL	0	NULL	VLA-4	GP		bind					VCAM-1	GP	endothelial			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_353_s_130	10669630	(3) Binding of monocyte VLA-4 by endothelial VCAM-1 is needed for the induction of IL-1beta in monocytes.	bind
4540	2	2340	6	10	NULL	0	NULL	statement 1	Process		induces					IL-1beta	GP				NULL	monocytes	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_353_s_130	10669630	(3) Binding of monocyte VLA-4 by endothelial VCAM-1 is needed for the induction of IL-1beta in monocytes.	bind
53036	3	2340	6	10	NULL	0	NULL	VLA-4	Cell		is a type of					monocyte	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_353_s_130	10669630	(3) Binding of monocyte VLA-4 by endothelial VCAM-1 is needed for the induction of IL-1beta in monocytes.	bind
4413	1	2341	5	10	NULL	0	NULL	PsbP	GP	chlamydomonas	bind		functionally			PS II	GP	spinach			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_5	16049780	(3) Both Chlamydomonas  PsbP and spinach PsbP functionally bound to spinach PS II in the presence  of spinach PsbO.	bind
4415	2	2341	5	10	NULL	0	NULL	statement 1	Process		in the presence of					PsbO	GP	spinach			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_5	16049780	(3) Both Chlamydomonas  PsbP and spinach PsbP functionally bound to spinach PS II in the presence  of spinach PsbO.	bind
4419	3	2341	5	10	NULL	0	NULL	PsbP	GP	spinach	bind		functionally			PS II	GP	spinach			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_5	16049780	(3) Both Chlamydomonas  PsbP and spinach PsbP functionally bound to spinach PS II in the presence  of spinach PsbO.	bind
4421	4	2341	5	10	NULL	0	NULL	statement 3	Process		in the presence of					PsbO	GP	spinach			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_5	16049780	(3) Both Chlamydomonas  PsbP and spinach PsbP functionally bound to spinach PS II in the presence  of spinach PsbO.	bind
4541	1	2341	6	10	NULL	0	NULL	PsbP	GP	Chlamydomonas	bind		functionaly			PS II	GP	spinach			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_5	16049780	(3) Both Chlamydomonas  PsbP and spinach PsbP functionally bound to spinach PS II in the presence  of spinach PsbO.	bind
4542	2	2341	6	10	NULL	0	NULL	PsbP	GP	spinach	bind		functionaly			PS II	GP	spinach			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_5	16049780	(3) Both Chlamydomonas  PsbP and spinach PsbP functionally bound to spinach PS II in the presence  of spinach PsbO.	bind
4543	3	2341	6	10	NULL	0	NULL	statement 1	Process		occurs in presence of					PsbO	GP	spinach			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_5	16049780	(3) Both Chlamydomonas  PsbP and spinach PsbP functionally bound to spinach PS II in the presence  of spinach PsbO.	bind
4544	4	2341	6	10	NULL	0	NULL	statement 2	Process		occurs in presence of					PsbO	GP	spinach			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_5	16049780	(3) Both Chlamydomonas  PsbP and spinach PsbP functionally bound to spinach PS II in the presence  of spinach PsbO.	bind
4423	1	2342	5	10	NULL	0	NULL	p19ARF	GP		bind			amino-terminal domain		Mdm2	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_18_2358_s_102	10995391	(3) Conversely, the amino-terminal domain of p19ARF, which binds to Mdm2, also appears to be important in ensuring the interaction of ARF with another target required for S phase entry.	bind
4424	2	2342	5	10	NULL	0	NULL	ARF	GP		interact with					target required for S phase entry					NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_18_2358_s_102	10995391	(3) Conversely, the amino-terminal domain of p19ARF, which binds to Mdm2, also appears to be important in ensuring the interaction of ARF with another target required for S phase entry.	bind
4426	3	2342	5	10	NULL	0	NULL	p19ARF	GP		ensures			amino-terminal domain		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_18_2358_s_102	10995391	(3) Conversely, the amino-terminal domain of p19ARF, which binds to Mdm2, also appears to be important in ensuring the interaction of ARF with another target required for S phase entry.	bind
4545	1	2342	6	10	NULL	0	NULL	p19ARF	GP		bind			amino-terminal domain		Mdm2	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_18_2358_s_102	10995391	(3) Conversely, the amino-terminal domain of p19ARF, which binds to Mdm2, also appears to be important in ensuring the interaction of ARF with another target required for S phase entry.	bind
4546	2	2342	6	10	NULL	0	NULL	ARF	GP		interacts					target required for S phase entry					NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_18_2358_s_102	10995391	(3) Conversely, the amino-terminal domain of p19ARF, which binds to Mdm2, also appears to be important in ensuring the interaction of ARF with another target required for S phase entry.	bind
4547	3	2342	6	10	NULL	0	NULL	p19ARF	GP		ensures			amino-terminal domain		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_18_2358_s_102	10995391	(3) Conversely, the amino-terminal domain of p19ARF, which binds to Mdm2, also appears to be important in ensuring the interaction of ARF with another target required for S phase entry.	bind
4427	1	2343	5	10	NULL	0	NULL	E2F1	GP		bind					TopBP1	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_18_6_673_s_284	15075294	(3) E2F1 binding to TopBP1 is induced by ATM-dependent phosphorylation of E2F1; E2F binding to pRb is inhibited by phosphorylation of pRb.	bind
4428	2	2343	5	10	NULL	0	NULL	E2F1	GP	phosphorylation	dependent on					ATM	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_18_6_673_s_284	15075294	(3) E2F1 binding to TopBP1 is induced by ATM-dependent phosphorylation of E2F1; E2F binding to pRb is inhibited by phosphorylation of pRb.	bind
4429	3	2343	5	10	NULL	0	NULL	statement 2	Process		induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_18_6_673_s_284	15075294	(3) E2F1 binding to TopBP1 is induced by ATM-dependent phosphorylation of E2F1; E2F binding to pRb is inhibited by phosphorylation of pRb.	bind
4430	4	2343	5	10	NULL	0	NULL	E2F	GP		bind					pRb	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_18_6_673_s_284	15075294	(3) E2F1 binding to TopBP1 is induced by ATM-dependent phosphorylation of E2F1; E2F binding to pRb is inhibited by phosphorylation of pRb.	bind
4431	5	2343	5	10	NULL	0	NULL	pRb	GP	phosphorylation	inhibit					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_18_6_673_s_284	15075294	(3) E2F1 binding to TopBP1 is induced by ATM-dependent phosphorylation of E2F1; E2F binding to pRb is inhibited by phosphorylation of pRb.	bind
4548	1	2343	6	10	NULL	0	NULL	E2F1	GP		bind					TopBP1	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_18_6_673_s_284	15075294	(3) E2F1 binding to TopBP1 is induced by ATM-dependent phosphorylation of E2F1; E2F binding to pRb is inhibited by phosphorylation of pRb.	bind
4549	2	2343	6	10	NULL	0	NULL	E2F1	GP	phosphorylation of	is dependent on					ATM	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_18_6_673_s_284	15075294	(3) E2F1 binding to TopBP1 is induced by ATM-dependent phosphorylation of E2F1; E2F binding to pRb is inhibited by phosphorylation of pRb.	bind
4550	3	2343	6	10	NULL	0	NULL	statement 2	Process		induces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_18_6_673_s_284	15075294	(3) E2F1 binding to TopBP1 is induced by ATM-dependent phosphorylation of E2F1; E2F binding to pRb is inhibited by phosphorylation of pRb.	bind
4551	4	2343	6	10	NULL	0	NULL	E2F	GP		bind					pRb	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_18_6_673_s_284	15075294	(3) E2F1 binding to TopBP1 is induced by ATM-dependent phosphorylation of E2F1; E2F binding to pRb is inhibited by phosphorylation of pRb.	bind
4552	5	2343	6	10	NULL	0	NULL	statement 4	Process		is inhibited by					pRb	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_18_6_673_s_284	15075294	(3) E2F1 binding to TopBP1 is induced by ATM-dependent phosphorylation of E2F1; E2F binding to pRb is inhibited by phosphorylation of pRb.	bind
4432	1	2344	5	10	NULL	0	NULL	fatty acids	Chemical		released from					triglyceride stores	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1504_1_70_s_183	11239486	(3) Fatty acids are released from the triglyceride stores and serve two functions: (3a) they are activated to acyl-CoA, then converted to acyl-carnitine and transported into the mitochondrial matrix where they will substrate for oxidation and (3b) free fatty acids bind to UCP1 to increase its proton conductance.	bind
4433	2	2344	5	10	NULL	0	NULL	fatty acids	Chemical		are activated to					acyl-CoA	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1504_1_70_s_183	11239486	(3) Fatty acids are released from the triglyceride stores and serve two functions: (3a) they are activated to acyl-CoA, then converted to acyl-carnitine and transported into the mitochondrial matrix where they will substrate for oxidation and (3b) free fatty acids bind to UCP1 to increase its proton conductance.	bind
4434	3	2344	5	10	NULL	0	NULL	statement 2	Process		converted to					acyl-carnitine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1504_1_70_s_183	11239486	(3) Fatty acids are released from the triglyceride stores and serve two functions: (3a) they are activated to acyl-CoA, then converted to acyl-carnitine and transported into the mitochondrial matrix where they will substrate for oxidation and (3b) free fatty acids bind to UCP1 to increase its proton conductance.	bind
4435	4	2344	5	10	NULL	0	NULL	statement 3	Process		transported to					mitochondrial matrix	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1504_1_70_s_183	11239486	(3) Fatty acids are released from the triglyceride stores and serve two functions: (3a) they are activated to acyl-CoA, then converted to acyl-carnitine and transported into the mitochondrial matrix where they will substrate for oxidation and (3b) free fatty acids bind to UCP1 to increase its proton conductance.	bind
4436	5	2344	5	10	NULL	0	NULL	statement 4	Process		substrate for					oxidation	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1504_1_70_s_183	11239486	(3) Fatty acids are released from the triglyceride stores and serve two functions: (3a) they are activated to acyl-CoA, then converted to acyl-carnitine and transported into the mitochondrial matrix where they will substrate for oxidation and (3b) free fatty acids bind to UCP1 to increase its proton conductance.	bind
4437	6	2344	5	10	NULL	0	NULL	fatty acids	Chemical	free	bind					UCP1	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1504_1_70_s_183	11239486	(3) Fatty acids are released from the triglyceride stores and serve two functions: (3a) they are activated to acyl-CoA, then converted to acyl-carnitine and transported into the mitochondrial matrix where they will substrate for oxidation and (3b) free fatty acids bind to UCP1 to increase its proton conductance.	bind
4438	7	2344	5	10	NULL	0	NULL	statement 6	Process		increase					proton conductance	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1504_1_70_s_183	11239486	(3) Fatty acids are released from the triglyceride stores and serve two functions: (3a) they are activated to acyl-CoA, then converted to acyl-carnitine and transported into the mitochondrial matrix where they will substrate for oxidation and (3b) free fatty acids bind to UCP1 to increase its proton conductance.	bind
4553	1	2344	6	10	NULL	0	NULL	fatty acids	Chemical		released from					triglyceride stores	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1504_1_70_s_183	11239486	(3) Fatty acids are released from the triglyceride stores and serve two functions: (3a) they are activated to acyl-CoA, then converted to acyl-carnitine and transported into the mitochondrial matrix where they will substrate for oxidation and (3b) free fatty acids bind to UCP1 to increase its proton conductance.	bind
4589	2	2344	6	10	NULL	0	NULL	fatty acids	Chemical		are activated to					acyl-CoA	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1504_1_70_s_183	11239486	(3) Fatty acids are released from the triglyceride stores and serve two functions: (3a) they are activated to acyl-CoA, then converted to acyl-carnitine and transported into the mitochondrial matrix where they will substrate for oxidation and (3b) free fatty acids bind to UCP1 to increase its proton conductance.	bind
4590	3	2344	6	10	NULL	0	NULL	Acyl-CoA	GP		is converted to					acyl-carnitine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1504_1_70_s_183	11239486	(3) Fatty acids are released from the triglyceride stores and serve two functions: (3a) they are activated to acyl-CoA, then converted to acyl-carnitine and transported into the mitochondrial matrix where they will substrate for oxidation and (3b) free fatty acids bind to UCP1 to increase its proton conductance.	bind
4591	4	2344	6	10	NULL	0	NULL	fatty acids	Chemical		transported to					mitochondrial matrix	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1504_1_70_s_183	11239486	(3) Fatty acids are released from the triglyceride stores and serve two functions: (3a) they are activated to acyl-CoA, then converted to acyl-carnitine and transported into the mitochondrial matrix where they will substrate for oxidation and (3b) free fatty acids bind to UCP1 to increase its proton conductance.	bind
4592	5	2344	6	10	NULL	0	NULL	statement 3	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1504_1_70_s_183	11239486	(3) Fatty acids are released from the triglyceride stores and serve two functions: (3a) they are activated to acyl-CoA, then converted to acyl-carnitine and transported into the mitochondrial matrix where they will substrate for oxidation and (3b) free fatty acids bind to UCP1 to increase its proton conductance.	bind
4593	6	2344	6	10	NULL	0	NULL	fatty acids	Chemical	free	bind					UCP1	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1504_1_70_s_183	11239486	(3) Fatty acids are released from the triglyceride stores and serve two functions: (3a) they are activated to acyl-CoA, then converted to acyl-carnitine and transported into the mitochondrial matrix where they will substrate for oxidation and (3b) free fatty acids bind to UCP1 to increase its proton conductance.	bind
4594	7	2344	6	10	NULL	0	NULL	UCP1	GP		conducts					protons	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1504_1_70_s_183	11239486	(3) Fatty acids are released from the triglyceride stores and serve two functions: (3a) they are activated to acyl-CoA, then converted to acyl-carnitine and transported into the mitochondrial matrix where they will substrate for oxidation and (3b) free fatty acids bind to UCP1 to increase its proton conductance.	bind
4655	8	2344	6	10	NULL	0	NULL	statement 6	Process		increases					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1504_1_70_s_183	11239486	(3) Fatty acids are released from the triglyceride stores and serve two functions: (3a) they are activated to acyl-CoA, then converted to acyl-carnitine and transported into the mitochondrial matrix where they will substrate for oxidation and (3b) free fatty acids bind to UCP1 to increase its proton conductance.	bind
4439	1	2345	5	10	NULL	0	NULL	GalR	GP		bind					gal DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_17_2273_s_23	11544184	(3) Finally, there is a tripartite cooperativity between GalR and HU in binding to  gal DNA; binding of HU to  hbs is absolutely dependent on binding of GalR dimers to both operators and HU binding, in turn, results in increasing the strength of GalR binding.	bind
4440	2	2345	5	10	NULL	0	NULL	HU	GP		bind					gal DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_17_2273_s_23	11544184	(3) Finally, there is a tripartite cooperativity between GalR and HU in binding to  gal DNA; binding of HU to  hbs is absolutely dependent on binding of GalR dimers to both operators and HU binding, in turn, results in increasing the strength of GalR binding.	bind
4441	3	2345	5	10	NULL	0	NULL	HU	GP		bind					hbs	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_17_2273_s_23	11544184	(3) Finally, there is a tripartite cooperativity between GalR and HU in binding to  gal DNA; binding of HU to  hbs is absolutely dependent on binding of GalR dimers to both operators and HU binding, in turn, results in increasing the strength of GalR binding.	bind
4442	4	2345	5	10	NULL	0	NULL	GalR dimers	GP		bind									operators	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_17_2273_s_23	11544184	(3) Finally, there is a tripartite cooperativity between GalR and HU in binding to  gal DNA; binding of HU to  hbs is absolutely dependent on binding of GalR dimers to both operators and HU binding, in turn, results in increasing the strength of GalR binding.	bind
4443	5	2345	5	10	NULL	0	NULL	statement 3	Process		dependent on					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_17_2273_s_23	11544184	(3) Finally, there is a tripartite cooperativity between GalR and HU in binding to  gal DNA; binding of HU to  hbs is absolutely dependent on binding of GalR dimers to both operators and HU binding, in turn, results in increasing the strength of GalR binding.	bind
4444	6	2345	5	10	NULL	0	NULL	statement 3	Process		increases					GalR	GP	strength of;;binding of			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_17_2273_s_23	11544184	(3) Finally, there is a tripartite cooperativity between GalR and HU in binding to  gal DNA; binding of HU to  hbs is absolutely dependent on binding of GalR dimers to both operators and HU binding, in turn, results in increasing the strength of GalR binding.	bind
5929	7	2345	5	10	NULL	0	NULL	statement 1	Process		occurs in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_17_2273_s_23	11544184	(3) Finally, there is a tripartite cooperativity between GalR and HU in binding to  gal DNA; binding of HU to  hbs is absolutely dependent on binding of GalR dimers to both operators and HU binding, in turn, results in increasing the strength of GalR binding.	bind
4656	1	2345	6	10	NULL	0	NULL	GalR	GP		bind					gal DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_17_2273_s_23	11544184	(3) Finally, there is a tripartite cooperativity between GalR and HU in binding to  gal DNA; binding of HU to  hbs is absolutely dependent on binding of GalR dimers to both operators and HU binding, in turn, results in increasing the strength of GalR binding.	bind
4657	2	2345	6	10	NULL	0	NULL	HU	GP		bind					gal DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_17_2273_s_23	11544184	(3) Finally, there is a tripartite cooperativity between GalR and HU in binding to  gal DNA; binding of HU to  hbs is absolutely dependent on binding of GalR dimers to both operators and HU binding, in turn, results in increasing the strength of GalR binding.	bind
4658	3	2345	6	10	NULL	0	NULL	GalR dimer	GP		bind									operators	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_17_2273_s_23	11544184	(3) Finally, there is a tripartite cooperativity between GalR and HU in binding to  gal DNA; binding of HU to  hbs is absolutely dependent on binding of GalR dimers to both operators and HU binding, in turn, results in increasing the strength of GalR binding.	bind
4659	4	2345	6	10	NULL	0	NULL	HU	GP		bind					hbs	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_17_2273_s_23	11544184	(3) Finally, there is a tripartite cooperativity between GalR and HU in binding to  gal DNA; binding of HU to  hbs is absolutely dependent on binding of GalR dimers to both operators and HU binding, in turn, results in increasing the strength of GalR binding.	bind
4660	5	2345	6	10	NULL	0	NULL	statement 4	Process		is dependent on					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_17_2273_s_23	11544184	(3) Finally, there is a tripartite cooperativity between GalR and HU in binding to  gal DNA; binding of HU to  hbs is absolutely dependent on binding of GalR dimers to both operators and HU binding, in turn, results in increasing the strength of GalR binding.	bind
4661	6	2345	6	10	NULL	0	NULL	statement 4	Process		increases					GalR	GP	strength of ;;binding of			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_17_2273_s_23	11544184	(3) Finally, there is a tripartite cooperativity between GalR and HU in binding to  gal DNA; binding of HU to  hbs is absolutely dependent on binding of GalR dimers to both operators and HU binding, in turn, results in increasing the strength of GalR binding.	bind
5746	7	2345	6	10	NULL	0	NULL	statement 1	Process		occurs in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_17_2273_s_23	11544184	(3) Finally, there is a tripartite cooperativity between GalR and HU in binding to  gal DNA; binding of HU to  hbs is absolutely dependent on binding of GalR dimers to both operators and HU binding, in turn, results in increasing the strength of GalR binding.	bind
4445	1	2346	5	10	NULL	0	NULL	Importin alpha	GP		bind								NLSs		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_169_3_415_s_292	15883195	(3) Importin alpha binds to the NLSs and mediates the nuclear import of myopodin (4).	bind
4446	3	2346	5	10	NULL	0	NULL	Importin alpha	GP		mediate					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_169_3_415_s_292	15883195	(3) Importin alpha binds to the NLSs and mediates the nuclear import of myopodin (4).	bind
46479	2	2346	5	10	NULL	0	NULL	myopodin	GP		imported to					nucleus	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_169_3_415_s_292	15883195	(3) Importin alpha binds to the NLSs and mediates the nuclear import of myopodin (4).	bind
4595	1	2346	6	10	NULL	0	NULL	Importin alpha	GP		bind								NLS		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_169_3_415_s_292	15883195	(3) Importin alpha binds to the NLSs and mediates the nuclear import of myopodin (4).	bind
4600	2	2346	6	10	NULL	0	NULL	myopodin	GP		imported					nucleus	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_169_3_415_s_292	15883195	(3) Importin alpha binds to the NLSs and mediates the nuclear import of myopodin (4).	bind
4601	3	2346	6	10	NULL	0	NULL	Importin alpha	GP		mediates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_169_3_415_s_292	15883195	(3) Importin alpha binds to the NLSs and mediates the nuclear import of myopodin (4).	bind
4447	1	2347	5	10	NULL	0	NULL	19S RP	GP		bind		directly			Sec61 channel	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_21_0_435_s_42	16212502	(3) In a third scenario, the 19S RP binds directly to the Sec61 channel  and extracts misfolded proteins from the ER.	bind
4448	3	2347	5	10	NULL	0	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_21_0_435_s_42	16212502	(3) In a third scenario, the 19S RP binds directly to the Sec61 channel  and extracts misfolded proteins from the ER.	bind
46480	2	2347	5	10	NULL	0	NULL	 misfolded proteins	GP		extracted from					ER	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_21_0_435_s_42	16212502	(3) In a third scenario, the 19S RP binds directly to the Sec61 channel  and extracts misfolded proteins from the ER.	bind
4703	1	2347	6	10	NULL	0	NULL	19S RP	GP		bind		directly			Sec61 channel	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_21_0_435_s_42	16212502	(3) In a third scenario, the 19S RP binds directly to the Sec61 channel  and extracts misfolded proteins from the ER.	bind
4704	2	2347	6	10	NULL	0	NULL	misfolded proteins	GP		are extracted from					ER	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_21_0_435_s_42	16212502	(3) In a third scenario, the 19S RP binds directly to the Sec61 channel  and extracts misfolded proteins from the ER.	bind
4705	3	2347	6	10	NULL	0	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_21_0_435_s_42	16212502	(3) In a third scenario, the 19S RP binds directly to the Sec61 channel  and extracts misfolded proteins from the ER.	bind
4449	1	2348	5	10	NULL	0	NULL	neuropilin-1	GP		bind					SEMA-3A	GP		semaphorin portion		NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_19_18_7870_s_238	10479689	(3) In contrast, neither the A nor the B domains of neuropilin-1 appear to be required for the binding of the semaphorin portion of SEMA-3A.	bind
4450	2	2348	5	10	NULL	0	NULL	neuropilin-1	GP		is not required for			A domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_19_18_7870_s_238	10479689	(3) In contrast, neither the A nor the B domains of neuropilin-1 appear to be required for the binding of the semaphorin portion of SEMA-3A.	bind
4451	3	2348	5	10	NULL	0	NULL	neuropilin-1	GP		is not required for			B domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_19_18_7870_s_238	10479689	(3) In contrast, neither the A nor the B domains of neuropilin-1 appear to be required for the binding of the semaphorin portion of SEMA-3A.	bind
4706	2	2348	6	10	NULL	0	NULL	neuropilin-1	GP		is not required for 			A domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_19_18_7870_s_238	10479689	(3) In contrast, neither the A nor the B domains of neuropilin-1 appear to be required for the binding of the semaphorin portion of SEMA-3A.	bind
4781	3	2348	6	10	NULL	0	NULL	neuropilin-1	GP		are not required for 			B domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_19_18_7870_s_238	10479689	(3) In contrast, neither the A nor the B domains of neuropilin-1 appear to be required for the binding of the semaphorin portion of SEMA-3A.	bind
53037	1	2348	6	10	NULL	0	NULL	neuropilin-1	GP		bind					SEMA-3A	GP		semaphorin portion		NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_19_18_7870_s_238	10479689	(3) In contrast, neither the A nor the B domains of neuropilin-1 appear to be required for the binding of the semaphorin portion of SEMA-3A.	bind
4452	1	2349	5	10	NULL	0	NULL	Kar9p	GP		bind					Myo2p	GP		globular tail		NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_20_0_559_s_241	15473852	(3) Kar9p also binds the globular tail of Myo2p (myosin-V).	bind
4453	2	2349	5	10	NULL	0	NULL	Myo2p	GP		is					myosin-V	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_20_0_559_s_241	15473852	(3) Kar9p also binds the globular tail of Myo2p (myosin-V).	bind
4782	1	2349	6	10	NULL	0	NULL	Kar9p	GP		bind					Myo2p	GP		globular tail 		NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_20_0_559_s_241	15473852	(3) Kar9p also binds the globular tail of Myo2p (myosin-V).	bind
46481	2	2349	6	10	NULL	0	NULL	Myo2p	GP		is					myosin-V	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_20_0_559_s_241	15473852	(3) Kar9p also binds the globular tail of Myo2p (myosin-V).	bind
4454	2	2350	5	10	NULL	0	NULL	GST-Nck	GP	purified	bind		directly	SH2		statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_oncogene_15_15_9362449_s_11	9362449	(3) Purified GST-Nck-SH2 binds directly to  the GAP-associated p62.	bind
46482	1	2350	5	10	NULL	0	NULL	GAP	GP		associate with					p62	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_oncogene_15_15_9362449_s_11	9362449	(3) Purified GST-Nck-SH2 binds directly to  the GAP-associated p62.	bind
4785	2	2350	6	10	NULL	0	NULL	GST-Nck	GP	purified	bind		directly	SH2 domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_oncogene_15_15_9362449_s_11	9362449	(3) Purified GST-Nck-SH2 binds directly to  the GAP-associated p62.	bind
46483	1	2350	6	10	NULL	0	NULL	GAP	GP		associate with					p62	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_oncogene_15_15_9362449_s_11	9362449	(3) Purified GST-Nck-SH2 binds directly to  the GAP-associated p62.	bind
4455	1	2351	5	10	NULL	0	NULL	band 3 dimers	GP	stabilized	bind		effectively			GAPDH	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1559_1_43_s_256	11825587	(3) Stabilized band 3 dimers can also effectively bind GAPDH.	bind
4786	1	2351	6	10	NULL	0	NULL	band 3 dimers	GP	stabilized	bind		effectively			GAPDH	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1559_1_43_s_256	11825587	(3) Stabilized band 3 dimers can also effectively bind GAPDH.	bind
4456	1	2352	5	10	NULL	0	NULL	p53	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_4_462_s_211	9472015	(3) Stimulation of p53 DNA binding by HMG-1 was two to threefold greater when p53 half sites were separated by 10, 15, or 30 bp than when they were adjacent (data not shown).	bind
4457	2	2352	5	10	NULL	0	NULL	HMG-1	GP		stimulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_4_462_s_211	9472015	(3) Stimulation of p53 DNA binding by HMG-1 was two to threefold greater when p53 half sites were separated by 10, 15, or 30 bp than when they were adjacent (data not shown).	bind
4788	1	2352	6	10	NULL	0	NULL	p53	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_4_462_s_211	9472015	(3) Stimulation of p53 DNA binding by HMG-1 was two to threefold greater when p53 half sites were separated by 10, 15, or 30 bp than when they were adjacent (data not shown).	bind
4789	2	2352	6	10	NULL	0	NULL	HMG-1	GP		stimulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_4_462_s_211	9472015	(3) Stimulation of p53 DNA binding by HMG-1 was two to threefold greater when p53 half sites were separated by 10, 15, or 30 bp than when they were adjacent (data not shown).	bind
4458	1	2353	5	10	NULL	0	NULL	PD98059	Chemical		supress					ERK-AP-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_545_s_143	15020252	(3) Suppression  of ERK-AP-1 by PD98059 or dominant-negative mutants of ERK did not affect the apoptosis-promoting  effect of MG132.	bind
4459	2	2353	5	10	NULL	0	NULL	ERK	GP	dominant-negative mutants	supress					ERK-AP-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_545_s_143	15020252	(3) Suppression  of ERK-AP-1 by PD98059 or dominant-negative mutants of ERK did not affect the apoptosis-promoting  effect of MG132.	bind
4460	4	2353	5	10	NULL	0	NULL	statement 1	Process		does not affect					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_545_s_143	15020252	(3) Suppression  of ERK-AP-1 by PD98059 or dominant-negative mutants of ERK did not affect the apoptosis-promoting  effect of MG132.	bind
4461	5	2353	5	10	NULL	0	NULL	statement 2	Process		does not affect					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_545_s_143	15020252	(3) Suppression  of ERK-AP-1 by PD98059 or dominant-negative mutants of ERK did not affect the apoptosis-promoting  effect of MG132.	bind
46484	3	2353	5	10	NULL	0	NULL	MG132	Chemical		promotes					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_545_s_143	15020252	(3) Suppression  of ERK-AP-1 by PD98059 or dominant-negative mutants of ERK did not affect the apoptosis-promoting  effect of MG132.	bind
4792	1	2353	6	10	NULL	0	NULL	PD98059	Chemical		suppresses					ERK-AP-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_545_s_143	15020252	(3) Suppression  of ERK-AP-1 by PD98059 or dominant-negative mutants of ERK did not affect the apoptosis-promoting  effect of MG132.	bind
4793	2	2353	6	10	NULL	0	NULL	MG132	Chemical		promotes					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_545_s_143	15020252	(3) Suppression  of ERK-AP-1 by PD98059 or dominant-negative mutants of ERK did not affect the apoptosis-promoting  effect of MG132.	bind
46881	3	2353	6	10	NULL	0	NULL	ERK	GP	dominant-negative mutant	suppress					 ERK-AP-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_545_s_143	15020252	(3) Suppression  of ERK-AP-1 by PD98059 or dominant-negative mutants of ERK did not affect the apoptosis-promoting  effect of MG132.	bind
46882	4	2353	6	10	NULL	0	NULL	statement 1	Process		does not affect					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_545_s_143	15020252	(3) Suppression  of ERK-AP-1 by PD98059 or dominant-negative mutants of ERK did not affect the apoptosis-promoting  effect of MG132.	bind
53038	5	2353	6	10	NULL	0	NULL	statement 3	Process		does not affect					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_545_s_143	15020252	(3) Suppression  of ERK-AP-1 by PD98059 or dominant-negative mutants of ERK did not affect the apoptosis-promoting  effect of MG132.	bind
4463	1	2354	5	10	NULL	0	NULL	Mre11 protein	GP	mutant	bind					Rad50	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_95_5_705_s_74	9845372	(3) The  mre11-58 mutation inhibits  the complex formation by preventing binding of the mutant Mre11 protein to  Rad50 and Xrs2.	bind
4464	2	2354	5	10	NULL	0	NULL	Mre11 protein	GP	mutant	bind					Xrs2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_95_5_705_s_74	9845372	(3) The  mre11-58 mutation inhibits  the complex formation by preventing binding of the mutant Mre11 protein to  Rad50 and Xrs2.	bind
4465	3	2354	5	10	NULL	0	NULL	Mre11 protein	GP	mutation	prevent			mre11-58		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_95_5_705_s_74	9845372	(3) The  mre11-58 mutation inhibits  the complex formation by preventing binding of the mutant Mre11 protein to  Rad50 and Xrs2.	bind
4466	4	2354	5	10	NULL	0	NULL	Mre11 protein	GP	mutation	prevent			mre11-58		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_95_5_705_s_74	9845372	(3) The  mre11-58 mutation inhibits  the complex formation by preventing binding of the mutant Mre11 protein to  Rad50 and Xrs2.	bind
4467	5	2354	5	10	NULL	0	NULL	Mre11 protein	GP	mutation	inhibit			mre11-58		complex formation	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_95_5_705_s_74	9845372	(3) The  mre11-58 mutation inhibits  the complex formation by preventing binding of the mutant Mre11 protein to  Rad50 and Xrs2.	bind
4468	6	2354	5	10	NULL	0	NULL	statement 5	Process		occurs by					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_95_5_705_s_74	9845372	(3) The  mre11-58 mutation inhibits  the complex formation by preventing binding of the mutant Mre11 protein to  Rad50 and Xrs2.	bind
4469	7	2354	5	10	NULL	0	NULL	statement 5	Process		occurs by					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_95_5_705_s_74	9845372	(3) The  mre11-58 mutation inhibits  the complex formation by preventing binding of the mutant Mre11 protein to  Rad50 and Xrs2.	bind
4794	1	2354	6	10	NULL	0	NULL	Mre11 protein	GP		bind					Rad50	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_95_5_705_s_74	9845372	(3) The  mre11-58 mutation inhibits  the complex formation by preventing binding of the mutant Mre11 protein to  Rad50 and Xrs2.	bind
4795	2	2354	6	10	NULL	0	NULL	Mre11 protein	GP		bind					Xrs2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_95_5_705_s_74	9845372	(3) The  mre11-58 mutation inhibits  the complex formation by preventing binding of the mutant Mre11 protein to  Rad50 and Xrs2.	bind
4796	3	2354	6	10	NULL	0	NULL	Mre11 protein	GP	mutant	prevents			 mre11-58		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_95_5_705_s_74	9845372	(3) The  mre11-58 mutation inhibits  the complex formation by preventing binding of the mutant Mre11 protein to  Rad50 and Xrs2.	bind
4797	4	2354	6	10	NULL	0	NULL	Mre11 protein	GP	mutant	prevents			 mre11-58		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_95_5_705_s_74	9845372	(3) The  mre11-58 mutation inhibits  the complex formation by preventing binding of the mutant Mre11 protein to  Rad50 and Xrs2.	bind
4798	5	2354	6	10	NULL	0	NULL	Mre11 protein	GP	mutant	inhibits			 mre11-58		complex formation	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_95_5_705_s_74	9845372	(3) The  mre11-58 mutation inhibits  the complex formation by preventing binding of the mutant Mre11 protein to  Rad50 and Xrs2.	bind
53039	6	2354	6	10	NULL	0	NULL	statement 5	Process		occur by					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_95_5_705_s_74	9845372	(3) The  mre11-58 mutation inhibits  the complex formation by preventing binding of the mutant Mre11 protein to  Rad50 and Xrs2.	bind
53040	7	2354	6	10	NULL	0	NULL	statement 5	Process		occur by					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_95_5_705_s_74	9845372	(3) The  mre11-58 mutation inhibits  the complex formation by preventing binding of the mutant Mre11 protein to  Rad50 and Xrs2.	bind
4470	1	2356	5	10	NULL	0	NULL	RMP: RecO/Rad52/UvsY	GP		bind					SSB-ssDNA complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_24_15327_s_224	12438681	(3) The recombination mediator protein (RMP: RecO/Rad52/UvsY) binds to the SSB-ssDNA complex.	bind
4471	2	2356	5	10	NULL	0	NULL	RMP: RecO/Rad52/UvsY	GP		is					recombination mediator protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_24_15327_s_224	12438681	(3) The recombination mediator protein (RMP: RecO/Rad52/UvsY) binds to the SSB-ssDNA complex.	bind
4799	1	2356	6	10	NULL	0	NULL	RMP: RecO/Rad52/UvsY	GP		bind					SSB-ssDNA complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_24_15327_s_224	12438681	(3) The recombination mediator protein (RMP: RecO/Rad52/UvsY) binds to the SSB-ssDNA complex.	bind
4800	2	2356	6	10	NULL	0	NULL	RMP: RecO/Rad52/UvsY	GP		is					recombination mediator protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_24_15327_s_224	12438681	(3) The recombination mediator protein (RMP: RecO/Rad52/UvsY) binds to the SSB-ssDNA complex.	bind
4472	1	2357	5	10	NULL	0	NULL	PSA	GP		bind					HRP	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_zhejiang-da-xue-xue-bao-yi-xue-ban_34_5_16216051_s_7	16216051	(3) Three peptides (RMWSF, RYDYSY,  LRLRQL) were selectively synthesized, and different concentrations were  used to inhibit PSA and ConA binding to the HRP.	bind
4473	2	2357	5	10	NULL	0	NULL	ConA	GP		bind					HRP	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_zhejiang-da-xue-xue-bao-yi-xue-ban_34_5_16216051_s_7	16216051	(3) Three peptides (RMWSF, RYDYSY,  LRLRQL) were selectively synthesized, and different concentrations were  used to inhibit PSA and ConA binding to the HRP.	bind
4474	3	2357	5	10	NULL	0	NULL	RMWSF peptide	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_zhejiang-da-xue-xue-bao-yi-xue-ban_34_5_16216051_s_7	16216051	(3) Three peptides (RMWSF, RYDYSY,  LRLRQL) were selectively synthesized, and different concentrations were  used to inhibit PSA and ConA binding to the HRP.	bind
4475	4	2357	5	10	NULL	0	NULL	RMWSF peptide	GP		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_zhejiang-da-xue-xue-bao-yi-xue-ban_34_5_16216051_s_7	16216051	(3) Three peptides (RMWSF, RYDYSY,  LRLRQL) were selectively synthesized, and different concentrations were  used to inhibit PSA and ConA binding to the HRP.	bind
4476	5	2357	5	10	NULL	0	NULL	RYDYSY peptide	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_zhejiang-da-xue-xue-bao-yi-xue-ban_34_5_16216051_s_7	16216051	(3) Three peptides (RMWSF, RYDYSY,  LRLRQL) were selectively synthesized, and different concentrations were  used to inhibit PSA and ConA binding to the HRP.	bind
4477	6	2357	5	10	NULL	0	NULL	RYDYSY peptide	GP		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_zhejiang-da-xue-xue-bao-yi-xue-ban_34_5_16216051_s_7	16216051	(3) Three peptides (RMWSF, RYDYSY,  LRLRQL) were selectively synthesized, and different concentrations were  used to inhibit PSA and ConA binding to the HRP.	bind
4478	7	2357	5	10	NULL	0	NULL	LRLRQL peptide	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_zhejiang-da-xue-xue-bao-yi-xue-ban_34_5_16216051_s_7	16216051	(3) Three peptides (RMWSF, RYDYSY,  LRLRQL) were selectively synthesized, and different concentrations were  used to inhibit PSA and ConA binding to the HRP.	bind
4479	8	2357	5	10	NULL	0	NULL	LRLRQL peptide	GP		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_zhejiang-da-xue-xue-bao-yi-xue-ban_34_5_16216051_s_7	16216051	(3) Three peptides (RMWSF, RYDYSY,  LRLRQL) were selectively synthesized, and different concentrations were  used to inhibit PSA and ConA binding to the HRP.	bind
4801	1	2357	6	10	NULL	0	NULL	PSA	GP		bind					HRP	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_zhejiang-da-xue-xue-bao-yi-xue-ban_34_5_16216051_s_7	16216051	(3) Three peptides (RMWSF, RYDYSY,  LRLRQL) were selectively synthesized, and different concentrations were  used to inhibit PSA and ConA binding to the HRP.	bind
4802	2	2357	6	10	NULL	0	NULL	ConA	GP		bind					HRP	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_zhejiang-da-xue-xue-bao-yi-xue-ban_34_5_16216051_s_7	16216051	(3) Three peptides (RMWSF, RYDYSY,  LRLRQL) were selectively synthesized, and different concentrations were  used to inhibit PSA and ConA binding to the HRP.	bind
6458	3	2357	6	10	NULL	0	NULL	RMWSF peptide	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_zhejiang-da-xue-xue-bao-yi-xue-ban_34_5_16216051_s_7	16216051	(3) Three peptides (RMWSF, RYDYSY,  LRLRQL) were selectively synthesized, and different concentrations were  used to inhibit PSA and ConA binding to the HRP.	bind
6459	4	2357	6	10	NULL	0	NULL	RMWSF peptide	GP		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_zhejiang-da-xue-xue-bao-yi-xue-ban_34_5_16216051_s_7	16216051	(3) Three peptides (RMWSF, RYDYSY,  LRLRQL) were selectively synthesized, and different concentrations were  used to inhibit PSA and ConA binding to the HRP.	bind
6460	5	2357	6	10	NULL	0	NULL	RYDYSY peptide	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_zhejiang-da-xue-xue-bao-yi-xue-ban_34_5_16216051_s_7	16216051	(3) Three peptides (RMWSF, RYDYSY,  LRLRQL) were selectively synthesized, and different concentrations were  used to inhibit PSA and ConA binding to the HRP.	bind
6461	6	2357	6	10	NULL	0	NULL	RYDYSY peptide	GP		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_zhejiang-da-xue-xue-bao-yi-xue-ban_34_5_16216051_s_7	16216051	(3) Three peptides (RMWSF, RYDYSY,  LRLRQL) were selectively synthesized, and different concentrations were  used to inhibit PSA and ConA binding to the HRP.	bind
6462	7	2357	6	10	NULL	0	NULL	 LRLRQL peptide	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_zhejiang-da-xue-xue-bao-yi-xue-ban_34_5_16216051_s_7	16216051	(3) Three peptides (RMWSF, RYDYSY,  LRLRQL) were selectively synthesized, and different concentrations were  used to inhibit PSA and ConA binding to the HRP.	bind
6463	8	2357	6	10	NULL	0	NULL	 LRLRQL peptide	GP		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_zhejiang-da-xue-xue-bao-yi-xue-ban_34_5_16216051_s_7	16216051	(3) Three peptides (RMWSF, RYDYSY,  LRLRQL) were selectively synthesized, and different concentrations were  used to inhibit PSA and ConA binding to the HRP.	bind
4480	1	2358	5	10	NULL	0	NULL	 CbbR dimers	GP		bind					IR1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_4_1245_s_238	12562794	(3) Two CbbR dimers bound to IR1 and IR3, resulting in the bending of DNA at an angle of 64 degrees .	bind
4481	2	2358	5	10	NULL	0	NULL	 CbbR dimers	GP		bind					IR3	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_4_1245_s_238	12562794	(3) Two CbbR dimers bound to IR1 and IR3, resulting in the bending of DNA at an angle of 64 degrees .	bind
4482	3	2358	5	10	NULL	0	NULL	statement 1	Process		results in					DNA 	NucleicAcid	 bending of			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_4_1245_s_238	12562794	(3) Two CbbR dimers bound to IR1 and IR3, resulting in the bending of DNA at an angle of 64 degrees .	bind
4483	4	2358	5	10	NULL	0	NULL	statement 2	Process		results in					DNA	NucleicAcid	 bending of			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_4_1245_s_238	12562794	(3) Two CbbR dimers bound to IR1 and IR3, resulting in the bending of DNA at an angle of 64 degrees .	bind
4803	1	2358	6	10	NULL	0	NULL	CbbR dimer	GP		bind					IR1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_4_1245_s_238	12562794	(3) Two CbbR dimers bound to IR1 and IR3, resulting in the bending of DNA at an angle of 64 degrees .	bind
4804	2	2358	6	10	NULL	0	NULL	CbbR dimer	GP		bind					IR3	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_4_1245_s_238	12562794	(3) Two CbbR dimers bound to IR1 and IR3, resulting in the bending of DNA at an angle of 64 degrees .	bind
4805	3	2358	6	10	NULL	0	NULL	statement 1	Process		results in					DNA	NucleicAcid	bending of			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_4_1245_s_238	12562794	(3) Two CbbR dimers bound to IR1 and IR3, resulting in the bending of DNA at an angle of 64 degrees .	bind
4806	4	2358	6	10	NULL	0	NULL	statement 2	Process		results in					DNA	NucleicAcid	bending of			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_4_1245_s_238	12562794	(3) Two CbbR dimers bound to IR1 and IR3, resulting in the bending of DNA at an angle of 64 degrees .	bind
4484	1	2359	5	10	NULL	0	NULL	CbbR dimers	GP		bind					DNA	NucleicAcid			IR1 site	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_4_1245_s_238	12562794	(3) Two CbbR dimers bound to sites IR1 and IR2, relaxing the DNA bend by 9 degrees  to 55 degrees  in the presence of the CbbR inducer  NADPH.	bind
4485	2	2359	5	10	NULL	0	NULL	 CbbR dimers	GP		bind					DNA	NucleicAcid			IR2 site	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_4_1245_s_238	12562794	(3) Two CbbR dimers bound to sites IR1 and IR2, relaxing the DNA bend by 9 degrees  to 55 degrees  in the presence of the CbbR inducer  NADPH.	bind
4486	3	2359	5	10	NULL	0	NULL	statement 1	Process		relax					DNA bend	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_4_1245_s_238	12562794	(3) Two CbbR dimers bound to sites IR1 and IR2, relaxing the DNA bend by 9 degrees  to 55 degrees  in the presence of the CbbR inducer  NADPH.	bind
4487	4	2359	5	10	NULL	0	NULL	statement 2	Process		relax					DNA bend	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_4_1245_s_238	12562794	(3) Two CbbR dimers bound to sites IR1 and IR2, relaxing the DNA bend by 9 degrees  to 55 degrees  in the presence of the CbbR inducer  NADPH.	bind
4488	5	2359	5	10	NULL	0	NULL	statement 3	Process		in the presence of					NADPH	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_4_1245_s_238	12562794	(3) Two CbbR dimers bound to sites IR1 and IR2, relaxing the DNA bend by 9 degrees  to 55 degrees  in the presence of the CbbR inducer  NADPH.	bind
4489	6	2359	5	10	NULL	0	NULL	statement 4	Process		in the presence of					NADPH	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_4_1245_s_238	12562794	(3) Two CbbR dimers bound to sites IR1 and IR2, relaxing the DNA bend by 9 degrees  to 55 degrees  in the presence of the CbbR inducer  NADPH.	bind
46485	7	2359	5	10	NULL	0	NULL	NADPH	Chemical		is a type of					CbbR inducer	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_4_1245_s_238	12562794	(3) Two CbbR dimers bound to sites IR1 and IR2, relaxing the DNA bend by 9 degrees  to 55 degrees  in the presence of the CbbR inducer  NADPH.	bind
5005	1	2359	6	10	NULL	0	NULL	CbbR dimer	GP		bind					DNA	NucleicAcid			site IR1	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_4_1245_s_238	12562794	(3) Two CbbR dimers bound to sites IR1 and IR2, relaxing the DNA bend by 9 degrees  to 55 degrees  in the presence of the CbbR inducer  NADPH.	bind
5006	2	2359	6	10	NULL	0	NULL	CbbR dimer	GP		bind					DNA	NucleicAcid			site IR2	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_4_1245_s_238	12562794	(3) Two CbbR dimers bound to sites IR1 and IR2, relaxing the DNA bend by 9 degrees  to 55 degrees  in the presence of the CbbR inducer  NADPH.	bind
5007	3	2359	6	10	NULL	0	NULL	statement 1	Process		relaxes					DNA bend	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_4_1245_s_238	12562794	(3) Two CbbR dimers bound to sites IR1 and IR2, relaxing the DNA bend by 9 degrees  to 55 degrees  in the presence of the CbbR inducer  NADPH.	bind
5008	4	2359	6	10	NULL	0	NULL	statement 2	Process		relaxes					DNA bend	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_4_1245_s_238	12562794	(3) Two CbbR dimers bound to sites IR1 and IR2, relaxing the DNA bend by 9 degrees  to 55 degrees  in the presence of the CbbR inducer  NADPH.	bind
5009	5	2359	6	10	NULL	0	NULL	statement 3	Process		occurs in presence of					NADPH	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_4_1245_s_238	12562794	(3) Two CbbR dimers bound to sites IR1 and IR2, relaxing the DNA bend by 9 degrees  to 55 degrees  in the presence of the CbbR inducer  NADPH.	bind
5010	6	2359	6	10	NULL	0	NULL	statement 4	Process		occurs in presence of					NADPH	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_4_1245_s_238	12562794	(3) Two CbbR dimers bound to sites IR1 and IR2, relaxing the DNA bend by 9 degrees  to 55 degrees  in the presence of the CbbR inducer  NADPH.	bind
46486	7	2359	6	10	NULL	0	NULL	NADPH	Process		is a type of					CbbR inducer	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_4_1245_s_238	12562794	(3) Two CbbR dimers bound to sites IR1 and IR2, relaxing the DNA bend by 9 degrees  to 55 degrees  in the presence of the CbbR inducer  NADPH.	bind
4490	1	2360	5	10	NULL	0	NULL	CcpA	GP		bind		specifically			gnt gene	GP	B. subtilis		CRE	NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiolrev_19_3_187_s_129	9050218	(3) Using gel-retardation analysis, it was demonstrated that specific binding of CcpA to CRE of the  B. subtilis gnt gene is triggered by HPr(Ser-P) but not by free HPr.	bind
4491	2	2360	5	10	NULL	0	NULL	statement 1	Process		is triggered by					HPr	GP		Ser-P		NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiolrev_19_3_187_s_129	9050218	(3) Using gel-retardation analysis, it was demonstrated that specific binding of CcpA to CRE of the  B. subtilis gnt gene is triggered by HPr(Ser-P) but not by free HPr.	bind
4492	3	2360	5	10	NULL	0	NULL	statement 1	Process		is not triggered by					HPr	GP	free			NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiolrev_19_3_187_s_129	9050218	(3) Using gel-retardation analysis, it was demonstrated that specific binding of CcpA to CRE of the  B. subtilis gnt gene is triggered by HPr(Ser-P) but not by free HPr.	bind
5011	1	2360	6	10	NULL	0	NULL	CcpA	GP		bind		specifically			gnt gene	GP	B. subtilis		CRE	NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiolrev_19_3_187_s_129	9050218	(3) Using gel-retardation analysis, it was demonstrated that specific binding of CcpA to CRE of the  B. subtilis gnt gene is triggered by HPr(Ser-P) but not by free HPr.	bind
5012	2	2360	6	10	NULL	0	NULL	HPr	GP		triggers			Ser-P		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiolrev_19_3_187_s_129	9050218	(3) Using gel-retardation analysis, it was demonstrated that specific binding of CcpA to CRE of the  B. subtilis gnt gene is triggered by HPr(Ser-P) but not by free HPr.	bind
5013	3	2360	6	10	NULL	0	NULL	HPr	GP	free	does not trigger					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiolrev_19_3_187_s_129	9050218	(3) Using gel-retardation analysis, it was demonstrated that specific binding of CcpA to CRE of the  B. subtilis gnt gene is triggered by HPr(Ser-P) but not by free HPr.	bind
4493	1	2361	5	10	NULL	0	NULL	 permease	GP		bind			D55C		sugar co-substrate	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochem-biophys-res-commun_178_3_1872836_s_4	1872836	(3H) p-nitrophenyl-alpha-D-galactoside  (NPG) binding studies demonstrated that D55C permease binds the sugar  co-substrate but Na+ (or Li+) ions do no longer enhance the affinity of  D55C permease for the co-transported sugar.	bind
4494	2	2361	5	10	NULL	0	NULL	Na+ ions	Chemical		does not enhance					statement 1	Process	affinity of			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochem-biophys-res-commun_178_3_1872836_s_4	1872836	(3H) p-nitrophenyl-alpha-D-galactoside  (NPG) binding studies demonstrated that D55C permease binds the sugar  co-substrate but Na+ (or Li+) ions do no longer enhance the affinity of  D55C permease for the co-transported sugar.	bind
4495	3	2361	5	10	NULL	0	NULL	Li+ ions	Chemical		does not enhance					statement 1	Process	affinity of			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochem-biophys-res-commun_178_3_1872836_s_4	1872836	(3H) p-nitrophenyl-alpha-D-galactoside  (NPG) binding studies demonstrated that D55C permease binds the sugar  co-substrate but Na+ (or Li+) ions do no longer enhance the affinity of  D55C permease for the co-transported sugar.	bind
46487	4	2361	5	10	NULL	0	NULL	NPG	Chemical		is					p-nitrophenyl-alpha-D-galactoside	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochem-biophys-res-commun_178_3_1872836_s_4	1872836	(3H) p-nitrophenyl-alpha-D-galactoside  (NPG) binding studies demonstrated that D55C permease binds the sugar  co-substrate but Na+ (or Li+) ions do no longer enhance the affinity of  D55C permease for the co-transported sugar.	bind
46488	5	2361	5	10	NULL	0	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochem-biophys-res-commun_178_3_1872836_s_4	1872836	(3H) p-nitrophenyl-alpha-D-galactoside  (NPG) binding studies demonstrated that D55C permease binds the sugar  co-substrate but Na+ (or Li+) ions do no longer enhance the affinity of  D55C permease for the co-transported sugar.	bind
5014	1	2361	6	10	NULL	0	NULL	permease	GP		bind			D55C		sugar co-substrate	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochem-biophys-res-commun_178_3_1872836_s_4	1872836	(3H) p-nitrophenyl-alpha-D-galactoside  (NPG) binding studies demonstrated that D55C permease binds the sugar  co-substrate but Na+ (or Li+) ions do no longer enhance the affinity of  D55C permease for the co-transported sugar.	bind
5015	2	2361	6	10	NULL	0	NULL	NPG 	Chemical		is					p-nitrophenyl-alpha-D-galactoside	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochem-biophys-res-commun_178_3_1872836_s_4	1872836	(3H) p-nitrophenyl-alpha-D-galactoside  (NPG) binding studies demonstrated that D55C permease binds the sugar  co-substrate but Na+ (or Li+) ions do no longer enhance the affinity of  D55C permease for the co-transported sugar.	bind
5016	3	2361	6	10	NULL	0	NULL	Na+ ion	Chemical		do not enhance					statement 1	Process	affinity of			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochem-biophys-res-commun_178_3_1872836_s_4	1872836	(3H) p-nitrophenyl-alpha-D-galactoside  (NPG) binding studies demonstrated that D55C permease binds the sugar  co-substrate but Na+ (or Li+) ions do no longer enhance the affinity of  D55C permease for the co-transported sugar.	bind
5017	4	2361	6	10	NULL	0	NULL	Li+ ion	Chemical		do not enhance					statement 1	Process	affinity of			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochem-biophys-res-commun_178_3_1872836_s_4	1872836	(3H) p-nitrophenyl-alpha-D-galactoside  (NPG) binding studies demonstrated that D55C permease binds the sugar  co-substrate but Na+ (or Li+) ions do no longer enhance the affinity of  D55C permease for the co-transported sugar.	bind
5018	5	2361	6	10	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochem-biophys-res-commun_178_3_1872836_s_4	1872836	(3H) p-nitrophenyl-alpha-D-galactoside  (NPG) binding studies demonstrated that D55C permease binds the sugar  co-substrate but Na+ (or Li+) ions do no longer enhance the affinity of  D55C permease for the co-transported sugar.	bind
4496	1	2363	5	10	NULL	0	NULL	Src	GP	activated	bind					hDia2C	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_4_3_287_s_34	12636908	(4) Activated Src binds to hDia2C.	bind
5019	1	2363	6	10	NULL	0	NULL	Src	GP	activated	bind					hDia2C	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_4_3_287_s_34	12636908	(4) Activated Src binds to hDia2C.	bind
4497	1	2364	5	10	NULL	0	NULL	ATP	Chemical		bind					myosin	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_546_2_209_s_134	12832041	(4) ATP binding to the myosin causes the myosin to detach from the actin and change its structure (swinging back of the lever).	bind
4498	2	2364	5	10	NULL	0	NULL	myosin	GP		detaches from					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_546_2_209_s_134	12832041	(4) ATP binding to the myosin causes the myosin to detach from the actin and change its structure (swinging back of the lever).	bind
4499	3	2364	5	10	NULL	0	NULL	statement 1	Process		causes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_546_2_209_s_134	12832041	(4) ATP binding to the myosin causes the myosin to detach from the actin and change its structure (swinging back of the lever).	bind
4500	4	2364	5	10	NULL	0	NULL	statement 1	Process		causes					myosin	GP	structural change of			NULL		NULL	NULL	NULL	NULL	gw60_febslett_546_2_209_s_134	12832041	(4) ATP binding to the myosin causes the myosin to detach from the actin and change its structure (swinging back of the lever).	bind
5020	1	2364	6	10	NULL	0	NULL	ATP	Chemical		bind					myosin	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_546_2_209_s_134	12832041	(4) ATP binding to the myosin causes the myosin to detach from the actin and change its structure (swinging back of the lever).	bind
5021	2	2364	6	10	NULL	0	NULL	myosin	GP		detach from					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_546_2_209_s_134	12832041	(4) ATP binding to the myosin causes the myosin to detach from the actin and change its structure (swinging back of the lever).	bind
5022	3	2364	6	10	NULL	0	NULL	statement 1	Process		causes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_546_2_209_s_134	12832041	(4) ATP binding to the myosin causes the myosin to detach from the actin and change its structure (swinging back of the lever).	bind
5023	4	2364	6	10	NULL	0	NULL	statement 1	Process		causes					myosin	GP	structural change of			NULL		NULL	NULL	NULL	NULL	gw60_febslett_546_2_209_s_134	12832041	(4) ATP binding to the myosin causes the myosin to detach from the actin and change its structure (swinging back of the lever).	bind
4501	2	2365	5	10	NULL	0	NULL	statement 1	Process		downregulates during					adipogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_113_2_147_s_219	12705864	(4) Levels of active, GTP bound Rho are normally downregulated during the course of adipogenesis.	bind
46489	1	2365	5	10	NULL	0	NULL	GTP	Chemical		bind					Rho	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_113_2_147_s_219	12705864	(4) Levels of active, GTP bound Rho are normally downregulated during the course of adipogenesis.	bind
5025	1	2365	6	10	NULL	0	NULL	GTP	Chemical		bind					Rho	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_113_2_147_s_219	12705864	(4) Levels of active, GTP bound Rho are normally downregulated during the course of adipogenesis.	bind
5026	2	2365	6	10	NULL	0	NULL	statement 1	Process		downregulates during					adipogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_113_2_147_s_219	12705864	(4) Levels of active, GTP bound Rho are normally downregulated during the course of adipogenesis.	bind
4502	1	2367	5	10	NULL	0	NULL	PsbP	GP	chlamydomonas	bind		functionally			PS II	GP	spinach			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_6	16049780	(4) While Chlamydomonas PsbP functionally bound to spinach  PS II in the presence of Chlamydomonas PsbO, spinach PsbP bound loosely  to spinach PS II in the presence of Chlamydomonas PsbO with no concomitant  restoration of oxygen evolution.	bind
4503	2	2367	5	10	NULL	0	NULL	statement 1	Process		in the presence of					PsbO	GP	chlamydomonas			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_6	16049780	(4) While Chlamydomonas PsbP functionally bound to spinach  PS II in the presence of Chlamydomonas PsbO, spinach PsbP bound loosely  to spinach PS II in the presence of Chlamydomonas PsbO with no concomitant  restoration of oxygen evolution.	bind
4504	3	2367	5	10	NULL	0	NULL	PsbP	GP	spinach	bind		loosely			PS II	GP	spinach			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_6	16049780	(4) While Chlamydomonas PsbP functionally bound to spinach  PS II in the presence of Chlamydomonas PsbO, spinach PsbP bound loosely  to spinach PS II in the presence of Chlamydomonas PsbO with no concomitant  restoration of oxygen evolution.	bind
4505	4	2367	5	10	NULL	0	NULL	statement 3	Process		in the presence of					PsbO	GP	chlamydomonas			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_6	16049780	(4) While Chlamydomonas PsbP functionally bound to spinach  PS II in the presence of Chlamydomonas PsbO, spinach PsbP bound loosely  to spinach PS II in the presence of Chlamydomonas PsbO with no concomitant  restoration of oxygen evolution.	bind
5027	1	2367	6	10	NULL	0	NULL	PsbP	GP	Chlamydomonas	bind					PS II	GP	spinach			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_6	16049780	(4) While Chlamydomonas PsbP functionally bound to spinach  PS II in the presence of Chlamydomonas PsbO, spinach PsbP bound loosely  to spinach PS II in the presence of Chlamydomonas PsbO with no concomitant  restoration of oxygen evolution.	bind
5028	2	2367	6	10	NULL	0	NULL	statement 1	Process		 in presence of					PsbO	GP	Chlamydomonas			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_6	16049780	(4) While Chlamydomonas PsbP functionally bound to spinach  PS II in the presence of Chlamydomonas PsbO, spinach PsbP bound loosely  to spinach PS II in the presence of Chlamydomonas PsbO with no concomitant  restoration of oxygen evolution.	bind
5029	3	2367	6	10	NULL	0	NULL	Psbp	GP	spinach	bind		loosely			PS II	GP	spinach			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_6	16049780	(4) While Chlamydomonas PsbP functionally bound to spinach  PS II in the presence of Chlamydomonas PsbO, spinach PsbP bound loosely  to spinach PS II in the presence of Chlamydomonas PsbO with no concomitant  restoration of oxygen evolution.	bind
5030	4	2367	6	10	NULL	0	NULL	statement 3	Process		 in presence of					PsbO	GP	Chlamydomonas			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_6	16049780	(4) While Chlamydomonas PsbP functionally bound to spinach  PS II in the presence of Chlamydomonas PsbO, spinach PsbP bound loosely  to spinach PS II in the presence of Chlamydomonas PsbO with no concomitant  restoration of oxygen evolution.	bind
4506	1	2369	5	10	NULL	0	NULL	PsbQ	GP	chlamydomonas	bind					PS II	GP	spinach			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_7	16049780	(5) Chlamydomonas PsbQ bound to spinach  PS II in the presence of Chlamydomonas PsbP and PsbO or spinach PsbO but  not to spinach PS II in the presence of spinach PsbP and Chlamydomonas  PsbO or spinach PsbO.	bind
4507	2	2369	5	10	NULL	0	NULL	statement 1	Process		in the presence of					PsbP	GP	chlamydomonas			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_7	16049780	(5) Chlamydomonas PsbQ bound to spinach  PS II in the presence of Chlamydomonas PsbP and PsbO or spinach PsbO but  not to spinach PS II in the presence of spinach PsbP and Chlamydomonas  PsbO or spinach PsbO.	bind
4508	3	2369	5	10	NULL	0	NULL	statement 1	Process		in the presence of					PsbO	GP	chlamydomonas			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_7	16049780	(5) Chlamydomonas PsbQ bound to spinach  PS II in the presence of Chlamydomonas PsbP and PsbO or spinach PsbO but  not to spinach PS II in the presence of spinach PsbP and Chlamydomonas  PsbO or spinach PsbO.	bind
4509	4	2369	5	10	NULL	0	NULL	statement 1	Process		in the presence of					PsbO	GP	spinach			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_7	16049780	(5) Chlamydomonas PsbQ bound to spinach  PS II in the presence of Chlamydomonas PsbP and PsbO or spinach PsbO but  not to spinach PS II in the presence of spinach PsbP and Chlamydomonas  PsbO or spinach PsbO.	bind
4510	5	2369	5	10	NULL	0	NULL	PsbQ	GP	chlamydomonas	does not bind					PS II	GP	spinach			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_7	16049780	(5) Chlamydomonas PsbQ bound to spinach  PS II in the presence of Chlamydomonas PsbP and PsbO or spinach PsbO but  not to spinach PS II in the presence of spinach PsbP and Chlamydomonas  PsbO or spinach PsbO.	bind
4511	6	2369	5	10	NULL	0	NULL	statement 5	Process		in the presence of					PsbP	GP	spinach			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_7	16049780	(5) Chlamydomonas PsbQ bound to spinach  PS II in the presence of Chlamydomonas PsbP and PsbO or spinach PsbO but  not to spinach PS II in the presence of spinach PsbP and Chlamydomonas  PsbO or spinach PsbO.	bind
4512	7	2369	5	10	NULL	0	NULL	statement 5	Process		in the presence of					PsbO	GP	chlamydomonas			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_7	16049780	(5) Chlamydomonas PsbQ bound to spinach  PS II in the presence of Chlamydomonas PsbP and PsbO or spinach PsbO but  not to spinach PS II in the presence of spinach PsbP and Chlamydomonas  PsbO or spinach PsbO.	bind
4513	8	2369	5	10	NULL	0	NULL	statement 5	Process		in the presence of					PsbO	GP	spinach			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_7	16049780	(5) Chlamydomonas PsbQ bound to spinach  PS II in the presence of Chlamydomonas PsbP and PsbO or spinach PsbO but  not to spinach PS II in the presence of spinach PsbP and Chlamydomonas  PsbO or spinach PsbO.	bind
53041	9	2369	5	10	NULL	0	NULL	statement 4	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_7	16049780	(5) Chlamydomonas PsbQ bound to spinach  PS II in the presence of Chlamydomonas PsbP and PsbO or spinach PsbO but  not to spinach PS II in the presence of spinach PsbP and Chlamydomonas  PsbO or spinach PsbO.	bind
53042	10	2369	5	10	NULL	0	NULL	statement 8	Process		is an alternative to					statement 7	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_7	16049780	(5) Chlamydomonas PsbQ bound to spinach  PS II in the presence of Chlamydomonas PsbP and PsbO or spinach PsbO but  not to spinach PS II in the presence of spinach PsbP and Chlamydomonas  PsbO or spinach PsbO.	bind
5031	1	2369	6	10	NULL	0	NULL	PsbQ	GP	Chlamydomonas	bind					PS II	GP	spinach			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_7	16049780	(5) Chlamydomonas PsbQ bound to spinach  PS II in the presence of Chlamydomonas PsbP and PsbO or spinach PsbO but  not to spinach PS II in the presence of spinach PsbP and Chlamydomonas  PsbO or spinach PsbO.	bind
5032	2	2369	6	10	NULL	0	NULL	statement 1	Process		occurs in presence of					PsbP	GP	Chlamydomonas			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_7	16049780	(5) Chlamydomonas PsbQ bound to spinach  PS II in the presence of Chlamydomonas PsbP and PsbO or spinach PsbO but  not to spinach PS II in the presence of spinach PsbP and Chlamydomonas  PsbO or spinach PsbO.	bind
5033	3	2369	6	10	NULL	0	NULL	statement 1	Process		occurs in presence of					PsbO	GP	Chlamydomonas			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_7	16049780	(5) Chlamydomonas PsbQ bound to spinach  PS II in the presence of Chlamydomonas PsbP and PsbO or spinach PsbO but  not to spinach PS II in the presence of spinach PsbP and Chlamydomonas  PsbO or spinach PsbO.	bind
5034	4	2369	6	10	NULL	0	NULL	statement 1	Process		occurs in presence of					PsbO	GP	spinach			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_7	16049780	(5) Chlamydomonas PsbQ bound to spinach  PS II in the presence of Chlamydomonas PsbP and PsbO or spinach PsbO but  not to spinach PS II in the presence of spinach PsbP and Chlamydomonas  PsbO or spinach PsbO.	bind
5035	5	2369	6	10	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_7	16049780	(5) Chlamydomonas PsbQ bound to spinach  PS II in the presence of Chlamydomonas PsbP and PsbO or spinach PsbO but  not to spinach PS II in the presence of spinach PsbP and Chlamydomonas  PsbO or spinach PsbO.	bind
5036	6	2369	6	10	NULL	0	NULL	PsbQ	GP	Chlamydomonas	does not bind					PS II	GP	spinach			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_7	16049780	(5) Chlamydomonas PsbQ bound to spinach  PS II in the presence of Chlamydomonas PsbP and PsbO or spinach PsbO but  not to spinach PS II in the presence of spinach PsbP and Chlamydomonas  PsbO or spinach PsbO.	bind
5037	7	2369	6	10	NULL	0	NULL	statement 6	Process		occurs in presence of					PsbP	GP	spinach			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_7	16049780	(5) Chlamydomonas PsbQ bound to spinach  PS II in the presence of Chlamydomonas PsbP and PsbO or spinach PsbO but  not to spinach PS II in the presence of spinach PsbP and Chlamydomonas  PsbO or spinach PsbO.	bind
5038	8	2369	6	10	NULL	0	NULL	statement 6	Process		occurs in presence of					PsbO	GP	Chlamydomonas			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_7	16049780	(5) Chlamydomonas PsbQ bound to spinach  PS II in the presence of Chlamydomonas PsbP and PsbO or spinach PsbO but  not to spinach PS II in the presence of spinach PsbP and Chlamydomonas  PsbO or spinach PsbO.	bind
5039	9	2369	6	10	NULL	0	NULL	statement 6	Process		occurs in presence of					PsbO	GP	spinach			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_7	16049780	(5) Chlamydomonas PsbQ bound to spinach  PS II in the presence of Chlamydomonas PsbP and PsbO or spinach PsbO but  not to spinach PS II in the presence of spinach PsbP and Chlamydomonas  PsbO or spinach PsbO.	bind
5040	10	2369	6	10	NULL	0	NULL	statement 8	Process		is an alternative to					statement 9	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_photosynth-res_84_1-3_16049780_s_7	16049780	(5) Chlamydomonas PsbQ bound to spinach  PS II in the presence of Chlamydomonas PsbP and PsbO or spinach PsbO but  not to spinach PS II in the presence of spinach PsbP and Chlamydomonas  PsbO or spinach PsbO.	bind
4878	1	2371	5	10	NULL	0	NULL	HGF variant	GP		bind					HGF-NK1 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_429_1_1_s_79	9657372	(5) The  Kd values of HGF or MSP variants that bind to receptor (HGF-NK1, HGF-NK2, pro-HGF, MSP   chain) are 2-10-fold higher than the  Kds of the mature intact ligands.	bind
4879	2	2371	5	10	NULL	0	NULL	HGF variant	GP		bind					HGF-NK2 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_429_1_1_s_79	9657372	(5) The  Kd values of HGF or MSP variants that bind to receptor (HGF-NK1, HGF-NK2, pro-HGF, MSP   chain) are 2-10-fold higher than the  Kds of the mature intact ligands.	bind
4880	3	2371	5	10	NULL	0	NULL	HGF variant	GP		bind					pro-HGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_429_1_1_s_79	9657372	(5) The  Kd values of HGF or MSP variants that bind to receptor (HGF-NK1, HGF-NK2, pro-HGF, MSP   chain) are 2-10-fold higher than the  Kds of the mature intact ligands.	bind
4881	4	2371	5	10	NULL	0	NULL	HGF variant	GP		bind					MSP chain	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_429_1_1_s_79	9657372	(5) The  Kd values of HGF or MSP variants that bind to receptor (HGF-NK1, HGF-NK2, pro-HGF, MSP   chain) are 2-10-fold higher than the  Kds of the mature intact ligands.	bind
46699	5	2371	5	10	NULL	0	NULL	MSP variant	GP		bind					HGF-NK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_429_1_1_s_79	9657372	(5) The  Kd values of HGF or MSP variants that bind to receptor (HGF-NK1, HGF-NK2, pro-HGF, MSP   chain) are 2-10-fold higher than the  Kds of the mature intact ligands.	bind
46700	9	2371	5	10	NULL	0	NULL	statement 1	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_429_1_1_s_79	9657372	(5) The  Kd values of HGF or MSP variants that bind to receptor (HGF-NK1, HGF-NK2, pro-HGF, MSP   chain) are 2-10-fold higher than the  Kds of the mature intact ligands.	bind
46701	6	2371	5	10	NULL	0	NULL	MSP variant	GP		bind					HGF-NK2	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_429_1_1_s_79	9657372	(5) The  Kd values of HGF or MSP variants that bind to receptor (HGF-NK1, HGF-NK2, pro-HGF, MSP   chain) are 2-10-fold higher than the  Kds of the mature intact ligands.	bind
46702	10	2371	5	10	NULL	0	NULL	statement 2	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_429_1_1_s_79	9657372	(5) The  Kd values of HGF or MSP variants that bind to receptor (HGF-NK1, HGF-NK2, pro-HGF, MSP   chain) are 2-10-fold higher than the  Kds of the mature intact ligands.	bind
46703	7	2371	5	10	NULL	0	NULL	MSP variant	GP		bind					pro-HGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_429_1_1_s_79	9657372	(5) The  Kd values of HGF or MSP variants that bind to receptor (HGF-NK1, HGF-NK2, pro-HGF, MSP   chain) are 2-10-fold higher than the  Kds of the mature intact ligands.	bind
46704	8	2371	5	10	NULL	0	NULL	MSP variant	GP		bind					MSP chain	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_429_1_1_s_79	9657372	(5) The  Kd values of HGF or MSP variants that bind to receptor (HGF-NK1, HGF-NK2, pro-HGF, MSP   chain) are 2-10-fold higher than the  Kds of the mature intact ligands.	bind
46705	11	2371	5	10	NULL	0	NULL	statement 3	Process		is an alternative to					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_429_1_1_s_79	9657372	(5) The  Kd values of HGF or MSP variants that bind to receptor (HGF-NK1, HGF-NK2, pro-HGF, MSP   chain) are 2-10-fold higher than the  Kds of the mature intact ligands.	bind
46706	12	2371	5	10	NULL	0	NULL	statement 4	Process		is an alternative to					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_429_1_1_s_79	9657372	(5) The  Kd values of HGF or MSP variants that bind to receptor (HGF-NK1, HGF-NK2, pro-HGF, MSP   chain) are 2-10-fold higher than the  Kds of the mature intact ligands.	bind
5042	1	2371	6	10	NULL	0	NULL	HGF variant	GP		bind					HGF-NK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_429_1_1_s_79	9657372	(5) The  Kd values of HGF or MSP variants that bind to receptor (HGF-NK1, HGF-NK2, pro-HGF, MSP   chain) are 2-10-fold higher than the  Kds of the mature intact ligands.	bind
5043	2	2371	6	10	NULL	0	NULL	HGF variant	GP		bind					HGF-NK2	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_429_1_1_s_79	9657372	(5) The  Kd values of HGF or MSP variants that bind to receptor (HGF-NK1, HGF-NK2, pro-HGF, MSP   chain) are 2-10-fold higher than the  Kds of the mature intact ligands.	bind
5044	3	2371	6	10	NULL	0	NULL	HGF variant	GP		bind					pro-HGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_429_1_1_s_79	9657372	(5) The  Kd values of HGF or MSP variants that bind to receptor (HGF-NK1, HGF-NK2, pro-HGF, MSP   chain) are 2-10-fold higher than the  Kds of the mature intact ligands.	bind
5045	4	2371	6	10	NULL	0	NULL	HGF variant	GP		bind					MSP chain	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_429_1_1_s_79	9657372	(5) The  Kd values of HGF or MSP variants that bind to receptor (HGF-NK1, HGF-NK2, pro-HGF, MSP   chain) are 2-10-fold higher than the  Kds of the mature intact ligands.	bind
5046	5	2371	6	10	NULL	0	NULL	MSP variant	GP		bind					HGF-NK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_429_1_1_s_79	9657372	(5) The  Kd values of HGF or MSP variants that bind to receptor (HGF-NK1, HGF-NK2, pro-HGF, MSP   chain) are 2-10-fold higher than the  Kds of the mature intact ligands.	bind
5047	6	2371	6	10	NULL	0	NULL	MSP variant	GP		bind					HGF-NK2	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_429_1_1_s_79	9657372	(5) The  Kd values of HGF or MSP variants that bind to receptor (HGF-NK1, HGF-NK2, pro-HGF, MSP   chain) are 2-10-fold higher than the  Kds of the mature intact ligands.	bind
5048	7	2371	6	10	NULL	0	NULL	MSP variant	GP		bind					pro-HGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_429_1_1_s_79	9657372	(5) The  Kd values of HGF or MSP variants that bind to receptor (HGF-NK1, HGF-NK2, pro-HGF, MSP   chain) are 2-10-fold higher than the  Kds of the mature intact ligands.	bind
5049	8	2371	6	10	NULL	0	NULL	MSP variant	GP		bind					MSP chain	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_429_1_1_s_79	9657372	(5) The  Kd values of HGF or MSP variants that bind to receptor (HGF-NK1, HGF-NK2, pro-HGF, MSP   chain) are 2-10-fold higher than the  Kds of the mature intact ligands.	bind
5050	9	2371	6	10	NULL	0	NULL	statement 1	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_429_1_1_s_79	9657372	(5) The  Kd values of HGF or MSP variants that bind to receptor (HGF-NK1, HGF-NK2, pro-HGF, MSP   chain) are 2-10-fold higher than the  Kds of the mature intact ligands.	bind
5051	10	2371	6	10	NULL	0	NULL	statement 2	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_429_1_1_s_79	9657372	(5) The  Kd values of HGF or MSP variants that bind to receptor (HGF-NK1, HGF-NK2, pro-HGF, MSP   chain) are 2-10-fold higher than the  Kds of the mature intact ligands.	bind
5052	11	2371	6	10	NULL	0	NULL	statement 3	Process		is an alternative to					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_429_1_1_s_79	9657372	(5) The  Kd values of HGF or MSP variants that bind to receptor (HGF-NK1, HGF-NK2, pro-HGF, MSP   chain) are 2-10-fold higher than the  Kds of the mature intact ligands.	bind
5053	12	2371	6	10	NULL	0	NULL	statement 4	Process		is an alternative to					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_429_1_1_s_79	9657372	(5) The  Kd values of HGF or MSP variants that bind to receptor (HGF-NK1, HGF-NK2, pro-HGF, MSP   chain) are 2-10-fold higher than the  Kds of the mature intact ligands.	bind
4514	1	2372	5	10	NULL	0	NULL	eIF4GII	GP		bind			Leu					Trp-73		NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_6_707_s_153	10394359	(6) ( Leu in eIF4GII and  Met in 4E-BP1) binds to Trp-73, Leu-131, and Leu-135.	bind
4515	2	2372	5	10	NULL	0	NULL	eIF4GII	GP		bind			Leu					Leu-131		NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_6_707_s_153	10394359	(6) ( Leu in eIF4GII and  Met in 4E-BP1) binds to Trp-73, Leu-131, and Leu-135.	bind
4516	3	2372	5	10	NULL	0	NULL	eIF4GII	GP		bind			Leu					Leu-135		NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_6_707_s_153	10394359	(6) ( Leu in eIF4GII and  Met in 4E-BP1) binds to Trp-73, Leu-131, and Leu-135.	bind
4517	4	2372	5	10	NULL	0	NULL	4E-BP1	GP		bind			Met					Trp-73		NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_6_707_s_153	10394359	(6) ( Leu in eIF4GII and  Met in 4E-BP1) binds to Trp-73, Leu-131, and Leu-135.	bind
4518	5	2372	5	10	NULL	0	NULL	4E-BP1	GP		bind			Met					Leu-131		NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_6_707_s_153	10394359	(6) ( Leu in eIF4GII and  Met in 4E-BP1) binds to Trp-73, Leu-131, and Leu-135.	bind
4519	6	2372	5	10	NULL	0	NULL	4E-BP1	GP		bind			Met					Leu-135		NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_6_707_s_153	10394359	(6) ( Leu in eIF4GII and  Met in 4E-BP1) binds to Trp-73, Leu-131, and Leu-135.	bind
5054	1	2372	6	10	NULL	0	NULL	eIF4GII	GP		bind			Leu					Trp-73		NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_6_707_s_153	10394359	(6) ( Leu in eIF4GII and  Met in 4E-BP1) binds to Trp-73, Leu-131, and Leu-135.	bind
5055	2	2372	6	10	NULL	0	NULL	eIF4GII	GP		bind			Leu					Leu-131		NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_6_707_s_153	10394359	(6) ( Leu in eIF4GII and  Met in 4E-BP1) binds to Trp-73, Leu-131, and Leu-135.	bind
5056	3	2372	6	10	NULL	0	NULL	eIF4GII	GP		bind			Leu					Leu-135		NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_6_707_s_153	10394359	(6) ( Leu in eIF4GII and  Met in 4E-BP1) binds to Trp-73, Leu-131, and Leu-135.	bind
5057	4	2372	6	10	NULL	0	NULL	4E-BP1	GP		bind			Met					Trp-73		NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_6_707_s_153	10394359	(6) ( Leu in eIF4GII and  Met in 4E-BP1) binds to Trp-73, Leu-131, and Leu-135.	bind
5058	5	2372	6	10	NULL	0	NULL	4E-BP1	GP		bind			Met					Leu-131		NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_6_707_s_153	10394359	(6) ( Leu in eIF4GII and  Met in 4E-BP1) binds to Trp-73, Leu-131, and Leu-135.	bind
5059	6	2372	6	10	NULL	0	NULL	4E-BP1	GP		bind			Met					Leu-135		NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_6_707_s_153	10394359	(6) ( Leu in eIF4GII and  Met in 4E-BP1) binds to Trp-73, Leu-131, and Leu-135.	bind
4520	1	2375	5	10	NULL	0	NULL	E2F1	GP		bind					DP1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_8_2703_s_126	10436023	(7) E2F1 binds DP1.	bind
5060	1	2375	6	10	NULL	0	NULL	E2F1	GP		bind					DP1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_8_2703_s_126	10436023	(7) E2F1 binds DP1.	bind
4521	1	2376	5	10	NULL	0	NULL	ATP	Chemical		bind					actin	GP		subunit		NULL		NULL	NULL	NULL	NULL	gw60_cell_112_4_453_s_86	12600310	(8) Filaments age by hydrolysis of ATP bound to each actin subunit (white subunits turn yellow) followed by dissociation of the   phosphate (subunits turn red).	bind
4522	2	2376	5	10	NULL	0	NULL	filaments	CellComponent		age by					statement 1	Process	hydrolysis of			NULL		NULL	NULL	NULL	NULL	gw60_cell_112_4_453_s_86	12600310	(8) Filaments age by hydrolysis of ATP bound to each actin subunit (white subunits turn yellow) followed by dissociation of the   phosphate (subunits turn red).	bind
4523	3	2376	5	10	NULL	0	NULL	statement 2	Process		occurs following					phosphate	Chemical	dissociation of			NULL		NULL	NULL	NULL	NULL	gw60_cell_112_4_453_s_86	12600310	(8) Filaments age by hydrolysis of ATP bound to each actin subunit (white subunits turn yellow) followed by dissociation of the   phosphate (subunits turn red).	bind
5061	1	2376	6	10	NULL	0	NULL	ATP	Chemical		bind					actin subunit	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_4_453_s_86	12600310	(8) Filaments age by hydrolysis of ATP bound to each actin subunit (white subunits turn yellow) followed by dissociation of the   phosphate (subunits turn red).	bind
6568	2	2376	6	10	NULL	0	NULL	filaments 	CellComponent		age by					statement 1	Process	hydrolysis of			NULL		NULL	NULL	NULL	NULL	gw60_cell_112_4_453_s_86	12600310	(8) Filaments age by hydrolysis of ATP bound to each actin subunit (white subunits turn yellow) followed by dissociation of the   phosphate (subunits turn red).	bind
6569	3	2376	6	10	NULL	0	NULL	statement 2	Process		occurs following					phosphate	Chemical	dissociation of			NULL		NULL	NULL	NULL	NULL	gw60_cell_112_4_453_s_86	12600310	(8) Filaments age by hydrolysis of ATP bound to each actin subunit (white subunits turn yellow) followed by dissociation of the   phosphate (subunits turn red).	bind
4893	1	2377	5	10	NULL	0	NULL	H43 peptide	GP		does not bind		apparently			DnaK	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25668_s_118	11970958	(9-mers were derived from the overlap windows of DnaK-binding ( i.e. peptides H10, H18, H32, M18, and M39) or homologous ( i.e. peptides M10 and H39) regions; peptides H43 and H44 did not show apparent binding of DnaK, but were theoretically predicted to contain a DnaK-binding site (see Fig.  6).)	bind
4895	2	2377	5	10	NULL	0	NULL	H44 peptide	GP		does not bind		apparently			DnaK	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25668_s_118	11970958	(9-mers were derived from the overlap windows of DnaK-binding ( i.e. peptides H10, H18, H32, M18, and M39) or homologous ( i.e. peptides M10 and H39) regions; peptides H43 and H44 did not show apparent binding of DnaK, but were theoretically predicted to contain a DnaK-binding site (see Fig.  6).)	bind
4897	3	2377	5	10	NULL	0	NULL	H43 peptide	GP		contain		may						DnaK-binding site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25668_s_118	11970958	(9-mers were derived from the overlap windows of DnaK-binding ( i.e. peptides H10, H18, H32, M18, and M39) or homologous ( i.e. peptides M10 and H39) regions; peptides H43 and H44 did not show apparent binding of DnaK, but were theoretically predicted to contain a DnaK-binding site (see Fig.  6).)	bind
4899	4	2377	5	10	NULL	0	NULL	H44 peptide	GP		contain		may						DnaK-binding site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25668_s_118	11970958	(9-mers were derived from the overlap windows of DnaK-binding ( i.e. peptides H10, H18, H32, M18, and M39) or homologous ( i.e. peptides M10 and H39) regions; peptides H43 and H44 did not show apparent binding of DnaK, but were theoretically predicted to contain a DnaK-binding site (see Fig.  6).)	bind
5226	1	2377	6	10	NULL	0	NULL	peptide H43	GP		does not bind					DnaK	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25668_s_118	11970958	(9-mers were derived from the overlap windows of DnaK-binding ( i.e. peptides H10, H18, H32, M18, and M39) or homologous ( i.e. peptides M10 and H39) regions; peptides H43 and H44 did not show apparent binding of DnaK, but were theoretically predicted to contain a DnaK-binding site (see Fig.  6).)	bind
5227	2	2377	6	10	NULL	0	NULL	peptide H44	GP		does not bind					DnaK	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25668_s_118	11970958	(9-mers were derived from the overlap windows of DnaK-binding ( i.e. peptides H10, H18, H32, M18, and M39) or homologous ( i.e. peptides M10 and H39) regions; peptides H43 and H44 did not show apparent binding of DnaK, but were theoretically predicted to contain a DnaK-binding site (see Fig.  6).)	bind
5228	3	2377	6	10	NULL	0	NULL	peptide H43	GP		contain		may						DnaK-binding site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25668_s_118	11970958	(9-mers were derived from the overlap windows of DnaK-binding ( i.e. peptides H10, H18, H32, M18, and M39) or homologous ( i.e. peptides M10 and H39) regions; peptides H43 and H44 did not show apparent binding of DnaK, but were theoretically predicted to contain a DnaK-binding site (see Fig.  6).)	bind
5229	4	2377	6	10	NULL	0	NULL	peptide H44	GP		 contain		may						DnaK-binding site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25668_s_118	11970958	(9-mers were derived from the overlap windows of DnaK-binding ( i.e. peptides H10, H18, H32, M18, and M39) or homologous ( i.e. peptides M10 and H39) regions; peptides H43 and H44 did not show apparent binding of DnaK, but were theoretically predicted to contain a DnaK-binding site (see Fig.  6).)	bind
4904	1	2379	5	10	NULL	0	NULL	DNA	NucleicAcid		bind					ORC	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_166	12966094	(A - B1 - ) DNA bound to wild-type ORC in 5 mM or 5 muM ATP, respectively; 29 or 14 fmol of wild-type DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively, and 16 or 15 fmol of mutant DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively; 55 or 54 fmol of wild-type DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively, and 46 or 40 fmol of mutant DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively.	bind
4905	2	2379	5	10	NULL	0	NULL	statement 1	Process		in the presence of					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_166	12966094	(A - B1 - ) DNA bound to wild-type ORC in 5 mM or 5 muM ATP, respectively; 29 or 14 fmol of wild-type DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively, and 16 or 15 fmol of mutant DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively; 55 or 54 fmol of wild-type DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively, and 46 or 40 fmol of mutant DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively.	bind
4906	3	2379	5	10	NULL	0	NULL	DNA	NucleicAcid	wild-type	bind					ORC-1A	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_166	12966094	(A - B1 - ) DNA bound to wild-type ORC in 5 mM or 5 muM ATP, respectively; 29 or 14 fmol of wild-type DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively, and 16 or 15 fmol of mutant DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively; 55 or 54 fmol of wild-type DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively, and 46 or 40 fmol of mutant DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively.	bind
4907	4	2379	5	10	NULL	0	NULL	statement 2	Process		in the presence of					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_166	12966094	(A - B1 - ) DNA bound to wild-type ORC in 5 mM or 5 muM ATP, respectively; 29 or 14 fmol of wild-type DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively, and 16 or 15 fmol of mutant DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively; 55 or 54 fmol of wild-type DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively, and 46 or 40 fmol of mutant DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively.	bind
4908	5	2379	5	10	NULL	0	NULL	DNA	NucleicAcid	mutant	bind					ORC-1A	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_166	12966094	(A - B1 - ) DNA bound to wild-type ORC in 5 mM or 5 muM ATP, respectively; 29 or 14 fmol of wild-type DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively, and 16 or 15 fmol of mutant DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively; 55 or 54 fmol of wild-type DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively, and 46 or 40 fmol of mutant DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively.	bind
4909	6	2379	5	10	NULL	0	NULL	statement 5	Process		in the presence of					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_166	12966094	(A - B1 - ) DNA bound to wild-type ORC in 5 mM or 5 muM ATP, respectively; 29 or 14 fmol of wild-type DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively, and 16 or 15 fmol of mutant DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively; 55 or 54 fmol of wild-type DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively, and 46 or 40 fmol of mutant DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively.	bind
4911	7	2379	5	10	NULL	0	NULL	DNA	NucleicAcid	wild-type	bind					ORC-5A	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_166	12966094	(A - B1 - ) DNA bound to wild-type ORC in 5 mM or 5 muM ATP, respectively; 29 or 14 fmol of wild-type DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively, and 16 or 15 fmol of mutant DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively; 55 or 54 fmol of wild-type DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively, and 46 or 40 fmol of mutant DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively.	bind
4913	8	2379	5	10	NULL	0	NULL	statement 7	Process		in the presence of					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_166	12966094	(A - B1 - ) DNA bound to wild-type ORC in 5 mM or 5 muM ATP, respectively; 29 or 14 fmol of wild-type DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively, and 16 or 15 fmol of mutant DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively; 55 or 54 fmol of wild-type DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively, and 46 or 40 fmol of mutant DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively.	bind
4914	9	2379	5	10	NULL	0	NULL	DNA	NucleicAcid	mutant	bind					ORC-5A	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_166	12966094	(A - B1 - ) DNA bound to wild-type ORC in 5 mM or 5 muM ATP, respectively; 29 or 14 fmol of wild-type DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively, and 16 or 15 fmol of mutant DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively; 55 or 54 fmol of wild-type DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively, and 46 or 40 fmol of mutant DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively.	bind
4915	10	2379	5	10	NULL	0	NULL	statement 9	Process		in the presence of					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_166	12966094	(A - B1 - ) DNA bound to wild-type ORC in 5 mM or 5 muM ATP, respectively; 29 or 14 fmol of wild-type DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively, and 16 or 15 fmol of mutant DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively; 55 or 54 fmol of wild-type DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively, and 46 or 40 fmol of mutant DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively.	bind
5230	1	2379	6	10	NULL	0	NULL	DNA	NucleicAcid		bind					ORC	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_166	12966094	(A - B1 - ) DNA bound to wild-type ORC in 5 mM or 5 muM ATP, respectively; 29 or 14 fmol of wild-type DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively, and 16 or 15 fmol of mutant DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively; 55 or 54 fmol of wild-type DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively, and 46 or 40 fmol of mutant DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively.	bind
5231	2	2379	6	10	NULL	0	NULL	statement 1	Process		occurs in presence of					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_166	12966094	(A - B1 - ) DNA bound to wild-type ORC in 5 mM or 5 muM ATP, respectively; 29 or 14 fmol of wild-type DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively, and 16 or 15 fmol of mutant DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively; 55 or 54 fmol of wild-type DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively, and 46 or 40 fmol of mutant DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively.	bind
5232	3	2379	6	10	NULL	0	NULL	DNA	NucleicAcid	wild type	bind					ORC-1A	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_166	12966094	(A - B1 - ) DNA bound to wild-type ORC in 5 mM or 5 muM ATP, respectively; 29 or 14 fmol of wild-type DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively, and 16 or 15 fmol of mutant DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively; 55 or 54 fmol of wild-type DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively, and 46 or 40 fmol of mutant DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively.	bind
5233	4	2379	6	10	NULL	0	NULL	statement 3	Process		occurs in presence of					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_166	12966094	(A - B1 - ) DNA bound to wild-type ORC in 5 mM or 5 muM ATP, respectively; 29 or 14 fmol of wild-type DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively, and 16 or 15 fmol of mutant DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively; 55 or 54 fmol of wild-type DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively, and 46 or 40 fmol of mutant DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively.	bind
5234	5	2379	6	10	NULL	0	NULL	DNA	NucleicAcid	mutant	bind					ORC-1A	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_166	12966094	(A - B1 - ) DNA bound to wild-type ORC in 5 mM or 5 muM ATP, respectively; 29 or 14 fmol of wild-type DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively, and 16 or 15 fmol of mutant DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively; 55 or 54 fmol of wild-type DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively, and 46 or 40 fmol of mutant DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively.	bind
5235	6	2379	6	10	NULL	0	NULL	statement 5	Process		occurs in presence of					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_166	12966094	(A - B1 - ) DNA bound to wild-type ORC in 5 mM or 5 muM ATP, respectively; 29 or 14 fmol of wild-type DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively, and 16 or 15 fmol of mutant DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively; 55 or 54 fmol of wild-type DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively, and 46 or 40 fmol of mutant DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively.	bind
5236	7	2379	6	10	NULL	0	NULL	DNA	NucleicAcid	wild type	bind					ORC-5A	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_166	12966094	(A - B1 - ) DNA bound to wild-type ORC in 5 mM or 5 muM ATP, respectively; 29 or 14 fmol of wild-type DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively, and 16 or 15 fmol of mutant DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively; 55 or 54 fmol of wild-type DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively, and 46 or 40 fmol of mutant DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively.	bind
5237	8	2379	6	10	NULL	0	NULL	statement 7	Process		occurs in presence of					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_166	12966094	(A - B1 - ) DNA bound to wild-type ORC in 5 mM or 5 muM ATP, respectively; 29 or 14 fmol of wild-type DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively, and 16 or 15 fmol of mutant DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively; 55 or 54 fmol of wild-type DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively, and 46 or 40 fmol of mutant DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively.	bind
5238	9	2379	6	10	NULL	0	NULL	DNA	NucleicAcid	mutant	bind					ORC-5A	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_166	12966094	(A - B1 - ) DNA bound to wild-type ORC in 5 mM or 5 muM ATP, respectively; 29 or 14 fmol of wild-type DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively, and 16 or 15 fmol of mutant DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively; 55 or 54 fmol of wild-type DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively, and 46 or 40 fmol of mutant DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively.	bind
5239	10	2379	6	10	NULL	0	NULL	statement 9	Process		occurs in presence of					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_166	12966094	(A - B1 - ) DNA bound to wild-type ORC in 5 mM or 5 muM ATP, respectively; 29 or 14 fmol of wild-type DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively, and 16 or 15 fmol of mutant DNA bound to ORC-1A in 5 mM or 5 muM ATP, respectively; 55 or 54 fmol of wild-type DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively, and 46 or 40 fmol of mutant DNA bound to ORC-5A in 5 mM or 5 muM ATP, respectively.	bind
4925	1	2381	5	10	NULL	0	NULL	ADP	Chemical		dissociate from					acto-myosin complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_6_1263_s_184	12628919	(A - M) to weak binding (A + M - ATP) of acto-myosin follows ADP dissociation from acto-myosin complex and subsequent binding of ATP to myosin.	bind
4926	2	2381	5	10	NULL	0	NULL	ATP	Chemical		bind					myosin	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_6_1263_s_184	12628919	(A - M) to weak binding (A + M - ATP) of acto-myosin follows ADP dissociation from acto-myosin complex and subsequent binding of ATP to myosin.	bind
4927	3	2381	5	10	NULL	0	NULL	statement 2	Process		occurs following					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_6_1263_s_184	12628919	(A - M) to weak binding (A + M - ATP) of acto-myosin follows ADP dissociation from acto-myosin complex and subsequent binding of ATP to myosin.	bind
4928	4	2381	5	10	NULL	0	NULL	acto-myosin	GP	weak binding of	follows					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_6_1263_s_184	12628919	(A - M) to weak binding (A + M - ATP) of acto-myosin follows ADP dissociation from acto-myosin complex and subsequent binding of ATP to myosin.	bind
6564	1	2381	6	10	NULL	0	NULL	ADP	Chemical		dissociates from					acto-myosin complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_6_1263_s_184	12628919	(A - M) to weak binding (A + M - ATP) of acto-myosin follows ADP dissociation from acto-myosin complex and subsequent binding of ATP to myosin.	bind
6565	2	2381	6	10	NULL	0	NULL	ATP	Chemical		bind					myosin	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_6_1263_s_184	12628919	(A - M) to weak binding (A + M - ATP) of acto-myosin follows ADP dissociation from acto-myosin complex and subsequent binding of ATP to myosin.	bind
6566	3	2381	6	10	NULL	0	NULL	statement 2	Process		occurs following					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_6_1263_s_184	12628919	(A - M) to weak binding (A + M - ATP) of acto-myosin follows ADP dissociation from acto-myosin complex and subsequent binding of ATP to myosin.	bind
6567	4	2381	6	10	NULL	0	NULL	acto-myosin	GP	weak binding of	follows					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_6_1263_s_184	12628919	(A - M) to weak binding (A + M - ATP) of acto-myosin follows ADP dissociation from acto-myosin complex and subsequent binding of ATP to myosin.	bind
4929	1	2382	5	10	NULL	0	NULL	2 -NH3+ group	Chemical		deprotonates in					aqueous solution	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_7_2_85_s_75	10662698	(A 2 -NH3+ group deprotonates with a pKa of  6.2 in aqueous solution  [20]  ; the pKa of this group is even lower with rSN bound to the ribozyme, as described below.)	bind
4930	2	2382	5	10	NULL	0	NULL	rSN	NucleicAcid		bind					ribozyme	GP				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_7_2_85_s_75	10662698	(A 2 -NH3+ group deprotonates with a pKa of  6.2 in aqueous solution  [20]  ; the pKa of this group is even lower with rSN bound to the ribozyme, as described below.)	bind
5063	1	2382	6	10	NULL	0	NULL	rSN	NucleicAcid		bind					ribozyme	GP				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_7_2_85_s_75	10662698	(A 2 -NH3+ group deprotonates with a pKa of  6.2 in aqueous solution  [20]  ; the pKa of this group is even lower with rSN bound to the ribozyme, as described below.)	bind
53043	2	2382	6	10	NULL	0	NULL	2 -NH3+ group	Chemical		deprotonates in					aqueous solution	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_7_2_85_s_75	10662698	(A 2 -NH3+ group deprotonates with a pKa of  6.2 in aqueous solution  [20]  ; the pKa of this group is even lower with rSN bound to the ribozyme, as described below.)	bind
4554	1	2383	5	10	NULL	0	NULL	HDMEC	Cell		bind					TSP-1	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-invest-dermatol_106_2_8601718_s_10	8601718	(A 4.1 and C 6.1) failed to block HDMEC binding to TSP-1, but  both MoAbs inhibited G361 human melanoma cell binding to TSP-1 by 60%.	bind
4555	2	2383	5	10	NULL	0	NULL	A 4.1	GP		failed to block					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-invest-dermatol_106_2_8601718_s_10	8601718	(A 4.1 and C 6.1) failed to block HDMEC binding to TSP-1, but  both MoAbs inhibited G361 human melanoma cell binding to TSP-1 by 60%.	bind
4556	3	2383	5	10	NULL	0	NULL	C 6.1	GP		failed to block					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-invest-dermatol_106_2_8601718_s_10	8601718	(A 4.1 and C 6.1) failed to block HDMEC binding to TSP-1, but  both MoAbs inhibited G361 human melanoma cell binding to TSP-1 by 60%.	bind
4557	4	2383	5	10	NULL	0	NULL	G361	Cell		bind					TSP-1	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-invest-dermatol_106_2_8601718_s_10	8601718	(A 4.1 and C 6.1) failed to block HDMEC binding to TSP-1, but  both MoAbs inhibited G361 human melanoma cell binding to TSP-1 by 60%.	bind
4558	5	2383	5	10	NULL	0	NULL	A 4.1	GP		inhibit					statement 4	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-invest-dermatol_106_2_8601718_s_10	8601718	(A 4.1 and C 6.1) failed to block HDMEC binding to TSP-1, but  both MoAbs inhibited G361 human melanoma cell binding to TSP-1 by 60%.	bind
46697	6	2383	5	10	NULL	0	NULL	G361	Cell		is a type of					human melanoma cell	Cell				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-invest-dermatol_106_2_8601718_s_10	8601718	(A 4.1 and C 6.1) failed to block HDMEC binding to TSP-1, but  both MoAbs inhibited G361 human melanoma cell binding to TSP-1 by 60%.	bind
53044	7	2383	5	10	NULL	0	NULL	 C 6.1	GP		inhibit					statement 4	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-invest-dermatol_106_2_8601718_s_10	8601718	(A 4.1 and C 6.1) failed to block HDMEC binding to TSP-1, but  both MoAbs inhibited G361 human melanoma cell binding to TSP-1 by 60%.	bind
53045	8	2383	5	10	NULL	0	NULL	A 4.1	GP		is a type of					MoAbs	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-invest-dermatol_106_2_8601718_s_10	8601718	(A 4.1 and C 6.1) failed to block HDMEC binding to TSP-1, but  both MoAbs inhibited G361 human melanoma cell binding to TSP-1 by 60%.	bind
53046	9	2383	5	10	NULL	0	NULL	C 6.1	GP		is a type of					MoAbs	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-invest-dermatol_106_2_8601718_s_10	8601718	(A 4.1 and C 6.1) failed to block HDMEC binding to TSP-1, but  both MoAbs inhibited G361 human melanoma cell binding to TSP-1 by 60%.	bind
5064	1	2383	6	10	NULL	0	NULL	HDMEC	Cell		bind					TSP-1	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-invest-dermatol_106_2_8601718_s_10	8601718	(A 4.1 and C 6.1) failed to block HDMEC binding to TSP-1, but  both MoAbs inhibited G361 human melanoma cell binding to TSP-1 by 60%.	bind
5065	2	2383	6	10	NULL	0	NULL	A 4.1	GP		failed to block					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-invest-dermatol_106_2_8601718_s_10	8601718	(A 4.1 and C 6.1) failed to block HDMEC binding to TSP-1, but  both MoAbs inhibited G361 human melanoma cell binding to TSP-1 by 60%.	bind
5066	3	2383	6	10	NULL	0	NULL	C 6.1	GP		failed to block					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-invest-dermatol_106_2_8601718_s_10	8601718	(A 4.1 and C 6.1) failed to block HDMEC binding to TSP-1, but  both MoAbs inhibited G361 human melanoma cell binding to TSP-1 by 60%.	bind
5067	4	2383	6	10	NULL	0	NULL	G361 	Cell		bind					TSP-1	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-invest-dermatol_106_2_8601718_s_10	8601718	(A 4.1 and C 6.1) failed to block HDMEC binding to TSP-1, but  both MoAbs inhibited G361 human melanoma cell binding to TSP-1 by 60%.	bind
5068	5	2383	6	10	NULL	0	NULL	A 4.1	GP		inhibits					statement 4	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-invest-dermatol_106_2_8601718_s_10	8601718	(A 4.1 and C 6.1) failed to block HDMEC binding to TSP-1, but  both MoAbs inhibited G361 human melanoma cell binding to TSP-1 by 60%.	bind
5069	6	2383	6	10	NULL	0	NULL	C 6.1	GP		inhibits					statement 4	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-invest-dermatol_106_2_8601718_s_10	8601718	(A 4.1 and C 6.1) failed to block HDMEC binding to TSP-1, but  both MoAbs inhibited G361 human melanoma cell binding to TSP-1 by 60%.	bind
46698	7	2383	6	10	NULL	0	NULL	G361	Cell		is a type of					human melanoma cell	Cell				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-invest-dermatol_106_2_8601718_s_10	8601718	(A 4.1 and C 6.1) failed to block HDMEC binding to TSP-1, but  both MoAbs inhibited G361 human melanoma cell binding to TSP-1 by 60%.	bind
53047	8	2383	6	10	NULL	0	NULL	A 4.1	GP		is a type of					MoAbs	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-invest-dermatol_106_2_8601718_s_10	8601718	(A 4.1 and C 6.1) failed to block HDMEC binding to TSP-1, but  both MoAbs inhibited G361 human melanoma cell binding to TSP-1 by 60%.	bind
53048	9	2383	6	10	NULL	0	NULL	C 6.1	GP		is a type of					MoAbs	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-invest-dermatol_106_2_8601718_s_10	8601718	(A 4.1 and C 6.1) failed to block HDMEC binding to TSP-1, but  both MoAbs inhibited G361 human melanoma cell binding to TSP-1 by 60%.	bind
4559	1	2384	5	10	NULL	0	NULL	EspF	GP		bind		specifically			MBP-SNX9214	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_8_3110_s_65	16585770	(A and  B), but EspF bound specifically to MBP-SNX9214 and GST-SNX9FL (C).	bind
4560	2	2384	5	10	NULL	0	NULL	EspF	GP		bind		specifically			GST-SNX9FL	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_8_3110_s_65	16585770	(A and  B), but EspF bound specifically to MBP-SNX9214 and GST-SNX9FL (C).	bind
5070	1	2384	6	10	NULL	0	NULL	EspF	GP		bind		specifically			MBP-SNX9214	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_8_3110_s_65	16585770	(A and  B), but EspF bound specifically to MBP-SNX9214 and GST-SNX9FL (C).	bind
5071	2	2384	6	10	NULL	0	NULL	EspF	GP		bind		specifically			GST-SNX9FL	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_8_3110_s_65	16585770	(A and  B), but EspF bound specifically to MBP-SNX9214 and GST-SNX9FL (C).	bind
4561	1	2385	5	10	NULL	0	NULL	Wnt-5a	GP		activate					NLK	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_1_131_s_192	12482967	(A and B) Activation of NLK by Wnt-5a  is dependent on CaMKII and TAK1.	bind
4562	2	2385	5	10	NULL	0	NULL	statement 1	Process		is dependent on					CaMKII	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_1_131_s_192	12482967	(A and B) Activation of NLK by Wnt-5a  is dependent on CaMKII and TAK1.	bind
4563	3	2385	5	10	NULL	0	NULL	statement 1	Process		is dependent on					TAK1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_1_131_s_192	12482967	(A and B) Activation of NLK by Wnt-5a  is dependent on CaMKII and TAK1.	bind
5072	1	2385	6	10	NULL	0	NULL	Wnt-5a	GP		activates					NLK	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_1_131_s_192	12482967	(A and B) Activation of NLK by Wnt-5a  is dependent on CaMKII and TAK1.	bind
5073	2	2385	6	10	NULL	0	NULL	statement 1	Process		is dependent on					CaMKII	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_1_131_s_192	12482967	(A and B) Activation of NLK by Wnt-5a  is dependent on CaMKII and TAK1.	bind
5074	3	2385	6	10	NULL	0	NULL	statement 1	Process		is dependent on					TAK1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_1_131_s_192	12482967	(A and B) Activation of NLK by Wnt-5a  is dependent on CaMKII and TAK1.	bind
4564	1	2386	5	10	NULL	0	NULL	hOGG1	GP	wild-type	bind					DNA fragment	NucleicAcid	native		1234 bp	NULL		NULL	NULL	NULL	NULL	gw60_chembiol_9_3_345_s_84	11927259	(A and B) AFM images of wild-type hOGG1 bound to a 1234 bp native DNA fragment (no oxoG specifically introduced).	bind
5075	1	2386	6	10	NULL	0	NULL	hOGG1	GP	wild type	bind					DNA fragment	NucleicAcid	native		1234 bp 	NULL		NULL	NULL	NULL	NULL	gw60_chembiol_9_3_345_s_84	11927259	(A and B) AFM images of wild-type hOGG1 bound to a 1234 bp native DNA fragment (no oxoG specifically introduced).	bind
4565	1	2387	5	10	NULL	0	NULL	D1	GP		bind			ATP binding regions		ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_genetics_155_1_203_s_115	10790395	(A and B) Aligned sequences representing the ATP-binding regions of the D1	bind
5077	1	2387	6	10	NULL	0	NULL	D1	GP		bind			ATP binding regions		ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_genetics_155_1_203_s_115	10790395	(A and B) Aligned sequences representing the ATP-binding regions of the D1	bind
4566	1	2388	5	10	NULL	0	NULL	lactoferrin	GP	human	bind					D39	Organism				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_5_3372_s_220	11292760	(A and B) Binding of human and bovine lactoferrin and human transferrin to  S. pneumoniae D39 and EF3296.	bind
4567	2	2388	5	10	NULL	0	NULL	lactoferrin	GP	bovine	bind					D39	Organism				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_5_3372_s_220	11292760	(A and B) Binding of human and bovine lactoferrin and human transferrin to  S. pneumoniae D39 and EF3296.	bind
4568	3	2388	5	10	NULL	0	NULL	lactoferrin	GP	human	bind					EF3296	Organism				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_5_3372_s_220	11292760	(A and B) Binding of human and bovine lactoferrin and human transferrin to  S. pneumoniae D39 and EF3296.	bind
4569	4	2388	5	10	NULL	0	NULL	lactoferrin	GP	bovine	bind					EF3296	Organism				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_5_3372_s_220	11292760	(A and B) Binding of human and bovine lactoferrin and human transferrin to  S. pneumoniae D39 and EF3296.	bind
4570	5	2388	5	10	NULL	0	NULL	transferrin	GP	human	bind					D39	Organism				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_5_3372_s_220	11292760	(A and B) Binding of human and bovine lactoferrin and human transferrin to  S. pneumoniae D39 and EF3296.	bind
4571	6	2388	5	10	NULL	0	NULL	transferrin	GP	human	bind					EF3296	Organism				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_5_3372_s_220	11292760	(A and B) Binding of human and bovine lactoferrin and human transferrin to  S. pneumoniae D39 and EF3296.	bind
61103	7	2388	5	10	NULL	0	NULL	D39	Organism		is a strain of					S. pneumoniae	Organism				NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_5_3372_s_220	11292760	(A and B) Binding of human and bovine lactoferrin and human transferrin to  S. pneumoniae D39 and EF3296.	bind
61104	8	2388	5	10	NULL	0	NULL	EF3296	Organism		is a strain of					S. pneumoniae	Organism				NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_5_3372_s_220	11292760	(A and B) Binding of human and bovine lactoferrin and human transferrin to  S. pneumoniae D39 and EF3296.	bind
5078	1	2388	6	10	NULL	0	NULL	lactoferrin	GP	human	bind					D39	Organism				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_5_3372_s_220	11292760	(A and B) Binding of human and bovine lactoferrin and human transferrin to  S. pneumoniae D39 and EF3296.	bind
5079	2	2388	6	10	NULL	0	NULL	lactoferrin	GP	human	bind					EF3296	Organism				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_5_3372_s_220	11292760	(A and B) Binding of human and bovine lactoferrin and human transferrin to  S. pneumoniae D39 and EF3296.	bind
5080	3	2388	6	10	NULL	0	NULL	lactoferrin	GP	bovine	bind					D39	Organism				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_5_3372_s_220	11292760	(A and B) Binding of human and bovine lactoferrin and human transferrin to  S. pneumoniae D39 and EF3296.	bind
5081	4	2388	6	10	NULL	0	NULL	lactoferrin	GP	bovine	bind					EF3296	Organism				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_5_3372_s_220	11292760	(A and B) Binding of human and bovine lactoferrin and human transferrin to  S. pneumoniae D39 and EF3296.	bind
5082	5	2388	6	10	NULL	0	NULL	transferrin	GP	human	bind					D39	Organism				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_5_3372_s_220	11292760	(A and B) Binding of human and bovine lactoferrin and human transferrin to  S. pneumoniae D39 and EF3296.	bind
5083	6	2388	6	10	NULL	0	NULL	transferrin	GP	human	bind					EF3296	Organism				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_5_3372_s_220	11292760	(A and B) Binding of human and bovine lactoferrin and human transferrin to  S. pneumoniae D39 and EF3296.	bind
61105	8	2388	6	10	NULL	0	NULL	EF3296	Organism		is a strain of					S. pneumoniae	Organism				NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_5_3372_s_220	11292760	(A and B) Binding of human and bovine lactoferrin and human transferrin to  S. pneumoniae D39 and EF3296.	bind
61106	7	2388	6	10	NULL	0	NULL	D39	Organism		is a strain of					S. pneumoniae	Organism				NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_5_3372_s_220	11292760	(A and B) Binding of human and bovine lactoferrin and human transferrin to  S. pneumoniae D39 and EF3296.	bind
4931	1	2389	5	10	NULL	0	NULL	C3	GP		bind					bacteria	Organism				NULL	BALB/cByJ serum	NULL	NULL	NULL	NULL	gw70_infectimmun_71_1_218_s_236	12496169	(A and B) C3  bound to bacteria after opsonization in BALB/cByJ serum, detected by ELISA, as described  in Materials and Methods.	bind
5084	1	2389	6	10	NULL	0	NULL	C3	GP		bind					bacteria	Organism				NULL	BALB/cByJ serum	NULL	NULL	NULL	NULL	gw70_infectimmun_71_1_218_s_236	12496169	(A and B) C3  bound to bacteria after opsonization in BALB/cByJ serum, detected by ELISA, as described  in Materials and Methods.	bind
4933	1	2390	5	10	NULL	0	NULL	C3	GP		bind					bacteria	Organism				NULL	BALB/cByJ serum	NULL	NULL	NULL	NULL	gw60_infectimmun_71_1_218_s_236	12496169	(A and B) C3 bound to bacteria after opsonization in BALB/cByJ serum, detected by ELISA, as described in Materials and Methods.	bind
5086	1	2390	6	10	NULL	0	NULL	C3	GP		bind					bacteria	Organism				NULL	BALB/cByJ serum	NULL	NULL	NULL	NULL	gw60_infectimmun_71_1_218_s_236	12496169	(A and B) C3 bound to bacteria after opsonization in BALB/cByJ serum, detected by ELISA, as described in Materials and Methods.	bind
4938	1	2394	5	10	NULL	0	NULL	3E5 IgG1 MAb	GP		bind					GXM antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_3_1057_s_80	9488395	(A and B) ELISAs of 3E5 IgG (IgG1, IgG2a, IgG2b, and IgG3) and of 4H3 IgG (IgG1, IgG2b, and IgG3) MAb binding to GXM antigen, respectively; (C and D) competition assays.	bind
4939	2	2394	5	10	NULL	0	NULL	3E5 IgG2a MAb	GP		bind					GXM antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_3_1057_s_80	9488395	(A and B) ELISAs of 3E5 IgG (IgG1, IgG2a, IgG2b, and IgG3) and of 4H3 IgG (IgG1, IgG2b, and IgG3) MAb binding to GXM antigen, respectively; (C and D) competition assays.	bind
4940	3	2394	5	10	NULL	0	NULL	3E5 IgG2b MAb	GP		bind					GXM antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_3_1057_s_80	9488395	(A and B) ELISAs of 3E5 IgG (IgG1, IgG2a, IgG2b, and IgG3) and of 4H3 IgG (IgG1, IgG2b, and IgG3) MAb binding to GXM antigen, respectively; (C and D) competition assays.	bind
4941	4	2394	5	10	NULL	0	NULL	3E5 IgG3 MAb	GP		bind					GXM antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_3_1057_s_80	9488395	(A and B) ELISAs of 3E5 IgG (IgG1, IgG2a, IgG2b, and IgG3) and of 4H3 IgG (IgG1, IgG2b, and IgG3) MAb binding to GXM antigen, respectively; (C and D) competition assays.	bind
4943	5	2394	5	10	NULL	0	NULL	4H3 IgG1 MAb	GP		bind					GXM antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_3_1057_s_80	9488395	(A and B) ELISAs of 3E5 IgG (IgG1, IgG2a, IgG2b, and IgG3) and of 4H3 IgG (IgG1, IgG2b, and IgG3) MAb binding to GXM antigen, respectively; (C and D) competition assays.	bind
4944	6	2394	5	10	NULL	0	NULL	4H3 IgG2b MAb	GP		bind					GXM antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_3_1057_s_80	9488395	(A and B) ELISAs of 3E5 IgG (IgG1, IgG2a, IgG2b, and IgG3) and of 4H3 IgG (IgG1, IgG2b, and IgG3) MAb binding to GXM antigen, respectively; (C and D) competition assays.	bind
4945	7	2394	5	10	NULL	0	NULL	4H3 IgG3 MAb	GP		bind					GXM antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_3_1057_s_80	9488395	(A and B) ELISAs of 3E5 IgG (IgG1, IgG2a, IgG2b, and IgG3) and of 4H3 IgG (IgG1, IgG2b, and IgG3) MAb binding to GXM antigen, respectively; (C and D) competition assays.	bind
5088	1	2394	6	10	NULL	0	NULL	3E5 IgG1 MAb	GP		bind					GXM antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_3_1057_s_80	9488395	(A and B) ELISAs of 3E5 IgG (IgG1, IgG2a, IgG2b, and IgG3) and of 4H3 IgG (IgG1, IgG2b, and IgG3) MAb binding to GXM antigen, respectively; (C and D) competition assays.	bind
5089	2	2394	6	10	NULL	0	NULL	3E5 IgG2a MAb	GP		bind					GXM antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_3_1057_s_80	9488395	(A and B) ELISAs of 3E5 IgG (IgG1, IgG2a, IgG2b, and IgG3) and of 4H3 IgG (IgG1, IgG2b, and IgG3) MAb binding to GXM antigen, respectively; (C and D) competition assays.	bind
5090	3	2394	6	10	NULL	0	NULL	3E5 IgG2b MAb	GP		bind					GXM antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_3_1057_s_80	9488395	(A and B) ELISAs of 3E5 IgG (IgG1, IgG2a, IgG2b, and IgG3) and of 4H3 IgG (IgG1, IgG2b, and IgG3) MAb binding to GXM antigen, respectively; (C and D) competition assays.	bind
5091	4	2394	6	10	NULL	0	NULL	3E5 IgG3 MAb	GP		bind					GXM antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_3_1057_s_80	9488395	(A and B) ELISAs of 3E5 IgG (IgG1, IgG2a, IgG2b, and IgG3) and of 4H3 IgG (IgG1, IgG2b, and IgG3) MAb binding to GXM antigen, respectively; (C and D) competition assays.	bind
5092	5	2394	6	10	NULL	0	NULL	4H3 IgG1 MAb	GP		bind					GXM antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_3_1057_s_80	9488395	(A and B) ELISAs of 3E5 IgG (IgG1, IgG2a, IgG2b, and IgG3) and of 4H3 IgG (IgG1, IgG2b, and IgG3) MAb binding to GXM antigen, respectively; (C and D) competition assays.	bind
5093	6	2394	6	10	NULL	0	NULL	4H3 IgG2b MAb	GP		bind					GXM antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_3_1057_s_80	9488395	(A and B) ELISAs of 3E5 IgG (IgG1, IgG2a, IgG2b, and IgG3) and of 4H3 IgG (IgG1, IgG2b, and IgG3) MAb binding to GXM antigen, respectively; (C and D) competition assays.	bind
5094	7	2394	6	10	NULL	0	NULL	4H3 IgG3 MAb	GP		bind					GXM antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_3_1057_s_80	9488395	(A and B) ELISAs of 3E5 IgG (IgG1, IgG2a, IgG2b, and IgG3) and of 4H3 IgG (IgG1, IgG2b, and IgG3) MAb binding to GXM antigen, respectively; (C and D) competition assays.	bind
4572	1	2397	5	10	NULL	0	NULL	Gab2	GP		is recruited to					phagocytic cups	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_161_6_1151_s_172	12821647	(A and B) Gab2 recruitment to the phagocytic cups correlates with PIP3 binding to Gab2 PH domain.	bind
4573	2	2397	5	10	NULL	0	NULL	PIP3	GP		bind					Gab2	GP		PH domain		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_161_6_1151_s_172	12821647	(A and B) Gab2 recruitment to the phagocytic cups correlates with PIP3 binding to Gab2 PH domain.	bind
4574	3	2397	5	10	NULL	0	NULL	statement 1	Process		correlates with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_161_6_1151_s_172	12821647	(A and B) Gab2 recruitment to the phagocytic cups correlates with PIP3 binding to Gab2 PH domain.	bind
5095	1	2397	6	10	NULL	0	NULL	PIP3	GP		bind					Gab2	GP		PH domain		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_161_6_1151_s_172	12821647	(A and B) Gab2 recruitment to the phagocytic cups correlates with PIP3 binding to Gab2 PH domain.	bind
5096	2	2397	6	10	NULL	0	NULL	Gab2	GP		recruited					phagocytic cups	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_161_6_1151_s_172	12821647	(A and B) Gab2 recruitment to the phagocytic cups correlates with PIP3 binding to Gab2 PH domain.	bind
5097	3	2397	6	10	NULL	0	NULL	statement 2	Process		correlates with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_161_6_1151_s_172	12821647	(A and B) Gab2 recruitment to the phagocytic cups correlates with PIP3 binding to Gab2 PH domain.	bind
4575	1	2400	5	10	NULL	0	NULL	E2F	GP		bind					PIN1	GP			promoter	NULL	 breast cell lines	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_15_5281_s_170	12101225	(A and B) Levels of E2F binding to the  PIN1 promoter in different breast cell lines.	bind
5098	1	2400	6	10	NULL	0	NULL	E2F	GP		bind					PIN1	GP			promoter	NULL	breast cell line	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_15_5281_s_170	12101225	(A and B) Levels of E2F binding to the  PIN1 promoter in different breast cell lines.	bind
5099	2	2401	6	10	NULL	0	NULL	LXR/RXR heterodimer	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_6_2182_s_191	12612088	(A and B) LXR/RXR heterodimers bind to DR4 from the human PLTP promoter region.	bind
46250	1	2401	6	10	NULL	0	NULL				is present in				DR4	PLTP	GP	human		promoter region	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_6_2182_s_191	12612088	(A and B) LXR/RXR heterodimers bind to DR4 from the human PLTP promoter region.	bind
5606	2	2401	7	10	NULL	0	NULL	LXR/RXR heterodimers	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_6_2182_s_191	12612088	(A and B) LXR/RXR heterodimers bind to DR4 from the human PLTP promoter region.	bind
46249	1	2401	7	10	NULL	0	NULL				is present in				DR4	PLTP	GP	human		promoter region	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_6_2182_s_191	12612088	(A and B) LXR/RXR heterodimers bind to DR4 from the human PLTP promoter region.	bind
5100	1	2404	6	10	NULL	0	NULL	Akt1	GP	phosphorylated	bind			Thr-308		JIP1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_170_1_61_s_85	15998799	(A and B) shows that Akt1 phosphorylated on Thr-308 and that Ser-473 binds to JIP1.	bind
5101	2	2404	6	10	NULL	0	NULL	Akt1	GP	phosphorylated	bind			Ser-473		JIP1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_170_1_61_s_85	15998799	(A and B) shows that Akt1 phosphorylated on Thr-308 and that Ser-473 binds to JIP1.	bind
5607	1	2404	7	10	NULL	0	NULL	Akt1	GP	phosphorylated	bind			Thr-308		JIP1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_170_1_61_s_85	15998799	(A and B) shows that Akt1 phosphorylated on Thr-308 and that Ser-473 binds to JIP1.	bind
46251	2	2404	7	10	NULL	0	NULL	Akt1	GP	phosphorylated	bind			Ser-473		JIP1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_170_1_61_s_85	15998799	(A and B) shows that Akt1 phosphorylated on Thr-308 and that Ser-473 binds to JIP1.	bind
5102	1	2405	6	10	NULL	0	NULL	Akt1	GP		bind					SEK1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_170_1_61_s_217	15998799	(A and B) shows that binding of Akt1 to SEK1 gradually increased as a function of time during glucose deprivation without changes in the intracellular level of Akt1.	bind
5103	2	2405	6	10	NULL	0	NULL	glucose	Chemical	deprivation of	increases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_170_1_61_s_217	15998799	(A and B) shows that binding of Akt1 to SEK1 gradually increased as a function of time during glucose deprivation without changes in the intracellular level of Akt1.	bind
5105	3	2405	6	10	NULL	0	NULL	statement 2	Process		does not change					Akt1	GP	intracellular level of 			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_170_1_61_s_217	15998799	(A and B) shows that binding of Akt1 to SEK1 gradually increased as a function of time during glucose deprivation without changes in the intracellular level of Akt1.	bind
5608	1	2405	7	10	NULL	0	NULL	Akt1	GP		binds					SEK1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_170_1_61_s_217	15998799	(A and B) shows that binding of Akt1 to SEK1 gradually increased as a function of time during glucose deprivation without changes in the intracellular level of Akt1.	bind
5609	2	2405	7	10	NULL	0	NULL	statement 1	Process		increased during					glucose	Chemical	deprivation of			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_170_1_61_s_217	15998799	(A and B) shows that binding of Akt1 to SEK1 gradually increased as a function of time during glucose deprivation without changes in the intracellular level of Akt1.	bind
5610	3	2405	7	10	NULL	0	NULL	statement 2	Process		does not change					Akt1	GP	intracellular level of			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_170_1_61_s_217	15998799	(A and B) shows that binding of Akt1 to SEK1 gradually increased as a function of time during glucose deprivation without changes in the intracellular level of Akt1.	bind
5197	1	2406	6	10	NULL	0	NULL	SHP2	GP		bind					p97	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_2_6_729_s_219	9885561	(A and B) SHP2 binding to p97 is dispensable for IL-3-induced MAPK activation.	bind
5198	2	2406	6	10	NULL	0	NULL	IL-3	GP		induces					MAPK	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_2_6_729_s_219	9885561	(A and B) SHP2 binding to p97 is dispensable for IL-3-induced MAPK activation.	bind
5199	3	2406	6	10	NULL	0	NULL	statement 1	Process		is dispensable for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_2_6_729_s_219	9885561	(A and B) SHP2 binding to p97 is dispensable for IL-3-induced MAPK activation.	bind
5611	1	2406	7	10	NULL	0	NULL	SHP2	GP		bind					 p97	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_2_6_729_s_219	9885561	(A and B) SHP2 binding to p97 is dispensable for IL-3-induced MAPK activation.	bind
5612	2	2406	7	10	NULL	0	NULL	IL-3	GP		induce					MAPK	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_2_6_729_s_219	9885561	(A and B) SHP2 binding to p97 is dispensable for IL-3-induced MAPK activation.	bind
5613	3	2406	7	10	NULL	0	NULL	statement 1	Process		is dispensable for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_2_6_729_s_219	9885561	(A and B) SHP2 binding to p97 is dispensable for IL-3-induced MAPK activation.	bind
5200	1	2407	6	10	NULL	0	NULL	Snf2p	GP	myc-tagged	bind					ARG1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8829_s_77	14612422	(A and B) The  gcn4delta SNF2-myc (SY127) and  gcn4delta SNF5-myc (SY166) strains described in the legend to Fig.  1 were transformed with single-copy (s.c) plasmid p2382 or pSY285, harboring  GCN4-HA or  gcn4-14Ala-HA, respectively, or high-copy-number (h.c.) plasmid pHQ1303 or pHQ1304, harboring  GCN4 or  gcn4-14Ala, respectively, and subjected to ChIP analysis as described in the legend to Fig.   1 to measure binding of myc-tagged Snf2p or Snf5p to  ARG1	bind
5201	2	2407	6	10	NULL	0	NULL	Snf5p	GP	myc-tagged	bind					ARG1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8829_s_77	14612422	(A and B) The  gcn4delta SNF2-myc (SY127) and  gcn4delta SNF5-myc (SY166) strains described in the legend to Fig.  1 were transformed with single-copy (s.c) plasmid p2382 or pSY285, harboring  GCN4-HA or  gcn4-14Ala-HA, respectively, or high-copy-number (h.c.) plasmid pHQ1303 or pHQ1304, harboring  GCN4 or  gcn4-14Ala, respectively, and subjected to ChIP analysis as described in the legend to Fig.   1 to measure binding of myc-tagged Snf2p or Snf5p to  ARG1	bind
5202	3	2407	6	10	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8829_s_77	14612422	(A and B) The  gcn4delta SNF2-myc (SY127) and  gcn4delta SNF5-myc (SY166) strains described in the legend to Fig.  1 were transformed with single-copy (s.c) plasmid p2382 or pSY285, harboring  GCN4-HA or  gcn4-14Ala-HA, respectively, or high-copy-number (h.c.) plasmid pHQ1303 or pHQ1304, harboring  GCN4 or  gcn4-14Ala, respectively, and subjected to ChIP analysis as described in the legend to Fig.   1 to measure binding of myc-tagged Snf2p or Snf5p to  ARG1	bind
5614	1	2407	7	10	NULL	0	NULL	Snf2p	GP	myc-tagged	binds					ARG1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8829_s_77	14612422	(A and B) The  gcn4delta SNF2-myc (SY127) and  gcn4delta SNF5-myc (SY166) strains described in the legend to Fig.  1 were transformed with single-copy (s.c) plasmid p2382 or pSY285, harboring  GCN4-HA or  gcn4-14Ala-HA, respectively, or high-copy-number (h.c.) plasmid pHQ1303 or pHQ1304, harboring  GCN4 or  gcn4-14Ala, respectively, and subjected to ChIP analysis as described in the legend to Fig.   1 to measure binding of myc-tagged Snf2p or Snf5p to  ARG1	bind
5615	2	2407	7	10	NULL	0	NULL	Snf5p	GP	myc-tagged	binds					ARG1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8829_s_77	14612422	(A and B) The  gcn4delta SNF2-myc (SY127) and  gcn4delta SNF5-myc (SY166) strains described in the legend to Fig.  1 were transformed with single-copy (s.c) plasmid p2382 or pSY285, harboring  GCN4-HA or  gcn4-14Ala-HA, respectively, or high-copy-number (h.c.) plasmid pHQ1303 or pHQ1304, harboring  GCN4 or  gcn4-14Ala, respectively, and subjected to ChIP analysis as described in the legend to Fig.   1 to measure binding of myc-tagged Snf2p or Snf5p to  ARG1	bind
46252	3	2407	7	10	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8829_s_77	14612422	(A and B) The  gcn4delta SNF2-myc (SY127) and  gcn4delta SNF5-myc (SY166) strains described in the legend to Fig.  1 were transformed with single-copy (s.c) plasmid p2382 or pSY285, harboring  GCN4-HA or  gcn4-14Ala-HA, respectively, or high-copy-number (h.c.) plasmid pHQ1303 or pHQ1304, harboring  GCN4 or  gcn4-14Ala, respectively, and subjected to ChIP analysis as described in the legend to Fig.   1 to measure binding of myc-tagged Snf2p or Snf5p to  ARG1	bind
5203	2	2408	6	10	NULL	0	NULL	MeCP2	GP		bind					statement 1	Process				NULL	E11.5 cells	NULL	NULL	NULL	NULL	gw70_febslett_572_1_184_s_129	15304345	(A and B) The abundant binding of MeCP2 to the methylated   318 CpG site within the S100  gene promoter region in E11.5 cells.	bind
46253	1	2408	6	10	NULL	0	NULL			methylated	is present within				318 CpG site	S100 gene	GP			promoter region	NULL	E11.5 cells	NULL	NULL	NULL	NULL	gw70_febslett_572_1_184_s_129	15304345	(A and B) The abundant binding of MeCP2 to the methylated   318 CpG site within the S100  gene promoter region in E11.5 cells.	bind
5616	2	2408	7	10	NULL	0	NULL	MeCP2	GP		bind					statement 1	Process				NULL	E11.5 cells	NULL	NULL	NULL	NULL	gw70_febslett_572_1_184_s_129	15304345	(A and B) The abundant binding of MeCP2 to the methylated   318 CpG site within the S100  gene promoter region in E11.5 cells.	bind
46256	1	2408	7	10	NULL	0	NULL			methylated	is present within				318 CpG site	S100 gene	GP			promoter region	NULL	E11.5 cells	NULL	NULL	NULL	NULL	gw70_febslett_572_1_184_s_129	15304345	(A and B) The abundant binding of MeCP2 to the methylated   318 CpG site within the S100  gene promoter region in E11.5 cells.	bind
5204	1	2409	6	10	NULL	0	NULL	GFP-ssrA	GP	denatured	bind					GroEL trap	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_4_639_s_37	10882100	(A and B) The ClpX6 concentration was 0.3  M, the concentration of modified or unmodified ClpP14 was 1  M, and the concentration of GroEL14 trap was 10  M. Gel filtration experiments confirmed that denaturated GFP-ssrA was bound to the GroEL trap when the latter molecule was present (data not shown).	bind
5666	1	2409	7	10	NULL	0	NULL	GFP-ssrA	GP	denatured	binds					GroEL trap	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_4_639_s_37	10882100	(A and B) The ClpX6 concentration was 0.3  M, the concentration of modified or unmodified ClpP14 was 1  M, and the concentration of GroEL14 trap was 10  M. Gel filtration experiments confirmed that denaturated GFP-ssrA was bound to the GroEL trap when the latter molecule was present (data not shown).	bind
5205	1	2411	6	10	NULL	0	NULL	PDGF alpha receptor	GP		bind					PDGF chain	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_131_8_1546_s_21	11139430	(A and B), and two receptors for PDGF (alpha and beta) bind these two PDGF chains with different affinities (Claesson-Welsh, 1994  ).	bind
5206	2	2411	6	10	NULL	0	NULL	PDGF beta receptor	GP		bind					PDGF chain	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_131_8_1546_s_21	11139430	(A and B), and two receptors for PDGF (alpha and beta) bind these two PDGF chains with different affinities (Claesson-Welsh, 1994  ).	bind
5667	1	2411	7	10	NULL	0	NULL	PDGF alpha receptor	GP		bind					PDGF chain	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_131_8_1546_s_21	11139430	(A and B), and two receptors for PDGF (alpha and beta) bind these two PDGF chains with different affinities (Claesson-Welsh, 1994  ).	bind
5668	2	2411	7	10	NULL	0	NULL	PDGF beta receptor	GP		bind					PDGF chain	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_131_8_1546_s_21	11139430	(A and B), and two receptors for PDGF (alpha and beta) bind these two PDGF chains with different affinities (Claesson-Welsh, 1994  ).	bind
5671	3	2411	7	10	NULL	0	NULL	statement 1	Process	 affinity of	is different from					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_131_8_1546_s_21	11139430	(A and B), and two receptors for PDGF (alpha and beta) bind these two PDGF chains with different affinities (Claesson-Welsh, 1994  ).	bind
5210	1	2413	6	10	NULL	0	NULL	MT	CellComponent		bind			G-NM domain		MT	CellComponent	rhodamine labeled			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_1_46_s_245	13679510	(A and B, E and F) Micrographs of reconstituted Ran regulation of the MT binding  of the G-NM domain to rhodamine-labeled MTs. (C and D) Micrographs of NLS-2 MT binding  in the absence and presence of importin alpha/beta.	bind
5211	2	2413	6	10	NULL	0	NULL	Ran	GP		regulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_1_46_s_245	13679510	(A and B, E and F) Micrographs of reconstituted Ran regulation of the MT binding  of the G-NM domain to rhodamine-labeled MTs. (C and D) Micrographs of NLS-2 MT binding  in the absence and presence of importin alpha/beta.	bind
5673	1	2413	7	10	NULL	0	NULL	MT	GP		binds			G-NM domain		MTs	GP	rhodamine-labeled			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_1_46_s_245	13679510	(A and B, E and F) Micrographs of reconstituted Ran regulation of the MT binding  of the G-NM domain to rhodamine-labeled MTs. (C and D) Micrographs of NLS-2 MT binding  in the absence and presence of importin alpha/beta.	bind
5674	2	2413	7	10	NULL	0	NULL	Ran	GP		regulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_1_46_s_245	13679510	(A and B, E and F) Micrographs of reconstituted Ran regulation of the MT binding  of the G-NM domain to rhodamine-labeled MTs. (C and D) Micrographs of NLS-2 MT binding  in the absence and presence of importin alpha/beta.	bind
5215	1	2414	6	10	NULL	0	NULL	CLIC5	GP		bind		strongly			GST-ezrin	GP		475-586		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_5_1509_s_266	10793131	(A and B, lanes 4), we observed strong binding of CLIC5 and relatively low levels of CLIC4 binding to GST-ezrin 475-586.	bind
5216	2	2414	6	10	NULL	0	NULL	CLIC4	GP		bind		low 			GST-ezrin	GP		475-586		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_5_1509_s_266	10793131	(A and B, lanes 4), we observed strong binding of CLIC5 and relatively low levels of CLIC4 binding to GST-ezrin 475-586.	bind
5675	1	2414	7	10	NULL	0	NULL	CLIC5	GP		binds		strongly			GST-ezrin	GP		475-586		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_5_1509_s_266	10793131	(A and B, lanes 4), we observed strong binding of CLIC5 and relatively low levels of CLIC4 binding to GST-ezrin 475-586.	bind
5676	2	2414	7	10	NULL	0	NULL	CLIC4 	GP		binds		low level			GST-ezrin	GP		475-586		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_5_1509_s_266	10793131	(A and B, lanes 4), we observed strong binding of CLIC5 and relatively low levels of CLIC4 binding to GST-ezrin 475-586.	bind
5218	1	2416	6	10	NULL	0	NULL	ERalpha	GP		bind					pS2	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_10_3358_s_308	11971969	(A and C) The in vivo binding of ERalpha, AIB1, and ERAP140 to the pS2 promoter was examined by the ChIP assay.	bind
5219	2	2416	6	10	NULL	0	NULL	AIB1	GP		bind					pS2	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_10_3358_s_308	11971969	(A and C) The in vivo binding of ERalpha, AIB1, and ERAP140 to the pS2 promoter was examined by the ChIP assay.	bind
5220	3	2416	6	10	NULL	0	NULL	ERAP140	GP		bind					pS2	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_10_3358_s_308	11971969	(A and C) The in vivo binding of ERalpha, AIB1, and ERAP140 to the pS2 promoter was examined by the ChIP assay.	bind
5677	1	2416	7	10	NULL	0	NULL	ERalpha	GP		bind					pS2	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_10_3358_s_308	11971969	(A and C) The in vivo binding of ERalpha, AIB1, and ERAP140 to the pS2 promoter was examined by the ChIP assay.	bind
5678	2	2416	7	10	NULL	0	NULL	AIB1	GP		bind					pS2	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_10_3358_s_308	11971969	(A and C) The in vivo binding of ERalpha, AIB1, and ERAP140 to the pS2 promoter was examined by the ChIP assay.	bind
5679	3	2416	7	10	NULL	0	NULL	ERAP140	GP		bind					pS2	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_10_3358_s_308	11971969	(A and C) The in vivo binding of ERalpha, AIB1, and ERAP140 to the pS2 promoter was examined by the ChIP assay.	bind
5221	1	2417	6	10	NULL	0	NULL	membrin	GP		bind		efficiently			Arf-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_7_1039_s_121	15781476	(A and C), membrin efficiently bound to Arf-1 in the presence of the cross-linker.	bind
5222	2	2417	6	10	NULL	0	NULL	statement 1	Process		occurs in presence of					cross-linker					NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_7_1039_s_121	15781476	(A and C), membrin efficiently bound to Arf-1 in the presence of the cross-linker.	bind
5680	1	2417	7	10	NULL	0	NULL	membrin	GP		bind		efficiently			Arf-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_7_1039_s_121	15781476	(A and C), membrin efficiently bound to Arf-1 in the presence of the cross-linker.	bind
5681	2	2417	7	10	NULL	0	NULL	statement 1	Process		in the presence of					cross-linker					NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_7_1039_s_121	15781476	(A and C), membrin efficiently bound to Arf-1 in the presence of the cross-linker.	bind
5240	1	2418	6	10	NULL	0	NULL	bacteria	Organism		bind					rabbit anti- Shigella LPS antiserum					NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_11_6449_s_148	11035758	(A and E) Bacteria binding rabbit anti- Shigella LPS antiserum or goat anti-rabbit IgG conjugated with Texas red.	bind
5241	2	2418	6	10	NULL	0	NULL	bacteria	Organism		bind					goat anti-rabbit IgG	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_11_6449_s_148	11035758	(A and E) Bacteria binding rabbit anti- Shigella LPS antiserum or goat anti-rabbit IgG conjugated with Texas red.	bind
5682	1	2418	7	10	NULL	0	NULL	Bacteria	Organism		binds					rabbit anti- Shigella LPS antiserum					NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_11_6449_s_148	11035758	(A and E) Bacteria binding rabbit anti- Shigella LPS antiserum or goat anti-rabbit IgG conjugated with Texas red.	bind
5683	2	2418	7	10	NULL	0	NULL	Bacteria	Organism		bind					goat anti-rabbit IgG	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_11_6449_s_148	11035758	(A and E) Bacteria binding rabbit anti- Shigella LPS antiserum or goat anti-rabbit IgG conjugated with Texas red.	bind
5242	1	2419	6	10	NULL	0	NULL	TFIIIB	GP		bind		sequentially			RNA polymerase III	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_5_749_s_9	9660958	(A box and B box) are recognized directly by TFIIIC, which in turn directs sequential binding of TFIIIB and RNA polymerase III.	bind
5243	2	2419	6	10	NULL	0	NULL				is recognized by		directly		A box	TFIIIC	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_5_749_s_9	9660958	(A box and B box) are recognized directly by TFIIIC, which in turn directs sequential binding of TFIIIB and RNA polymerase III.	bind
5244	3	2419	6	10	NULL	0	NULL				is recognized by		directly		B box	TFIIIC	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_5_749_s_9	9660958	(A box and B box) are recognized directly by TFIIIC, which in turn directs sequential binding of TFIIIB and RNA polymerase III.	bind
5245	4	2419	6	10	NULL	0	NULL	statement 2	Process		directs					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_5_749_s_9	9660958	(A box and B box) are recognized directly by TFIIIC, which in turn directs sequential binding of TFIIIB and RNA polymerase III.	bind
5246	5	2419	6	10	NULL	0	NULL	statement 3	Process		directs					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_5_749_s_9	9660958	(A box and B box) are recognized directly by TFIIIC, which in turn directs sequential binding of TFIIIB and RNA polymerase III.	bind
5685	1	2419	7	10	NULL	0	NULL	TFIIIB	GP		bind		sequentially			RNA polymerase III	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_5_749_s_9	9660958	(A box and B box) are recognized directly by TFIIIC, which in turn directs sequential binding of TFIIIB and RNA polymerase III.	bind
5389	1	2420	6	10	NULL	0	NULL	ORF	NucleicAcid		bind				consensus sequence	ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_8_1995_s_152	9555878	(A consensus sequence or P loop), suggesting that the protein product of this ORF binds ATP or GTP ( 49,  58).	bind
5390	2	2420	6	10	NULL	0	NULL	ORF	NucleicAcid		bind				P loop	ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_8_1995_s_152	9555878	(A consensus sequence or P loop), suggesting that the protein product of this ORF binds ATP or GTP ( 49,  58).	bind
5391	3	2420	6	10	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_8_1995_s_152	9555878	(A consensus sequence or P loop), suggesting that the protein product of this ORF binds ATP or GTP ( 49,  58).	bind
5392	4	2420	6	10	NULL	0	NULL	ORF	NucleicAcid		bind				consensus sequence	GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_8_1995_s_152	9555878	(A consensus sequence or P loop), suggesting that the protein product of this ORF binds ATP or GTP ( 49,  58).	bind
5393	5	2420	6	10	NULL	0	NULL	ORF	NucleicAcid		bind				P loop	GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_8_1995_s_152	9555878	(A consensus sequence or P loop), suggesting that the protein product of this ORF binds ATP or GTP ( 49,  58).	bind
5394	6	2420	6	10	NULL	0	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_8_1995_s_152	9555878	(A consensus sequence or P loop), suggesting that the protein product of this ORF binds ATP or GTP ( 49,  58).	bind
5686	1	2420	7	10	NULL	0	NULL	ORF	NucleicAcid		binds				P loop	ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_8_1995_s_152	9555878	(A consensus sequence or P loop), suggesting that the protein product of this ORF binds ATP or GTP ( 49,  58).	bind
5687	2	2420	7	10	NULL	0	NULL	ORF	NucleicAcid		binds				P loop	GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_8_1995_s_152	9555878	(A consensus sequence or P loop), suggesting that the protein product of this ORF binds ATP or GTP ( 49,  58).	bind
5395	1	2421	6	10	NULL	0	NULL	GCP1	GP		bind					germ cell nuclear factors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_5056_s_146	9030569	(A instead of C), are required for maximal binding of GCP1 to germ cell nuclear factors.	bind
5688	1	2421	7	10	NULL	0	NULL	GCP1	GP		binds to					germ cell nuclear factors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_5056_s_146	9030569	(A instead of C), are required for maximal binding of GCP1 to germ cell nuclear factors.	bind
5396	1	2422	6	10	NULL	0	NULL	kinase anchor protein 79	GP		bind					PKC	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_23_3_788_s_270	12574407	(A kinase anchor protein 79) that binds both PKC and phosphatase 2B (Klauck et al., 1996  ) may be involved in the local regulation of phosphorylation cascades.	bind
5397	2	2422	6	10	NULL	0	NULL	kinase anchor protein 79	GP		bind					phosphatase 2B	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_23_3_788_s_270	12574407	(A kinase anchor protein 79) that binds both PKC and phosphatase 2B (Klauck et al., 1996  ) may be involved in the local regulation of phosphorylation cascades.	bind
5398	3	2422	6	10	NULL	0	NULL	kinase anchor protein 79	GP		regulate		may			phosphorylation cascade	Process				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_23_3_788_s_270	12574407	(A kinase anchor protein 79) that binds both PKC and phosphatase 2B (Klauck et al., 1996  ) may be involved in the local regulation of phosphorylation cascades.	bind
5689	1	2422	7	10	NULL	0	NULL	A kinase anchor protein 79	GP		binds to					PKC	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_23_3_788_s_270	12574407	(A kinase anchor protein 79) that binds both PKC and phosphatase 2B (Klauck et al., 1996  ) may be involved in the local regulation of phosphorylation cascades.	bind
5690	2	2422	7	10	NULL	0	NULL	A kinase anchor protein 79	GP		binds to					phosphatase 2B	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_23_3_788_s_270	12574407	(A kinase anchor protein 79) that binds both PKC and phosphatase 2B (Klauck et al., 1996  ) may be involved in the local regulation of phosphorylation cascades.	bind
5691	3	2422	7	10	NULL	0	NULL	A kinase anchor protein 79	GP		regulate		may			phosphorylation cascades	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_23_3_788_s_270	12574407	(A kinase anchor protein 79) that binds both PKC and phosphatase 2B (Klauck et al., 1996  ) may be involved in the local regulation of phosphorylation cascades.	bind
5430	1	2423	6	10	NULL	0	NULL	neutrophil specific decoy receptor	GP		is					Fc RIIIB	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_19_0_275_s_40	11244038	(A neutrophil specific decoy receptor, Fc RIIIB, is additionally found in humans  that binds IgG immune complexes without triggering activation.)	bind
5433	2	2423	6	10	NULL	0	NULL	Fc RIIIB	GP		bind					IgG immune complexes	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_19_0_275_s_40	11244038	(A neutrophil specific decoy receptor, Fc RIIIB, is additionally found in humans  that binds IgG immune complexes without triggering activation.)	bind
5435	3	2423	6	10	NULL	0	NULL	statement 2	Process		does not trigger					activation	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_19_0_275_s_40	11244038	(A neutrophil specific decoy receptor, Fc RIIIB, is additionally found in humans  that binds IgG immune complexes without triggering activation.)	bind
5692	1	2423	7	10	NULL	0	NULL	Fc RIIIB	GP	human	binds					IgG immune complexes	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_19_0_275_s_40	11244038	(A neutrophil specific decoy receptor, Fc RIIIB, is additionally found in humans  that binds IgG immune complexes without triggering activation.)	bind
5693	2	2423	7	10	NULL	0	NULL	Fc RIIIB	GP		is					neutrophil specific decoy receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_19_0_275_s_40	11244038	(A neutrophil specific decoy receptor, Fc RIIIB, is additionally found in humans  that binds IgG immune complexes without triggering activation.)	bind
5694	3	2423	7	10	NULL	0	NULL	statement 1	Process		does not trigger					activation	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_19_0_275_s_40	11244038	(A neutrophil specific decoy receptor, Fc RIIIB, is additionally found in humans  that binds IgG immune complexes without triggering activation.)	bind
5438	1	2425	6	10	NULL	0	NULL	PP2Ac	GP		bind		alternatively						alpha-4 subunit		NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_279_37_15252037_s_4	15252037	(A subunit or PR65); however, PP2Ac alternatively binds to alpha-4,  a subunit related to yeast Tap42 protein, which also associates with phosphatases  PP4 or PP6.	bind
5439	2	2425	6	10	NULL	0	NULL	alpha-4 subunit	GP		is related to					Tap42 protein	GP	yeast			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_279_37_15252037_s_4	15252037	(A subunit or PR65); however, PP2Ac alternatively binds to alpha-4,  a subunit related to yeast Tap42 protein, which also associates with phosphatases  PP4 or PP6.	bind
5441	3	2425	6	10	NULL	0	NULL	Tap42 protein	GP	yeast	associate					PP4	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_279_37_15252037_s_4	15252037	(A subunit or PR65); however, PP2Ac alternatively binds to alpha-4,  a subunit related to yeast Tap42 protein, which also associates with phosphatases  PP4 or PP6.	bind
5442	4	2425	6	10	NULL	0	NULL	Tap42 protein	GP	yeast	associate					PP6	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_279_37_15252037_s_4	15252037	(A subunit or PR65); however, PP2Ac alternatively binds to alpha-4,  a subunit related to yeast Tap42 protein, which also associates with phosphatases  PP4 or PP6.	bind
5443	5	2425	6	10	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_279_37_15252037_s_4	15252037	(A subunit or PR65); however, PP2Ac alternatively binds to alpha-4,  a subunit related to yeast Tap42 protein, which also associates with phosphatases  PP4 or PP6.	bind
46258	6	2425	6	10	NULL	0	NULL	PP4	GP		is a type of					phosphatases	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_279_37_15252037_s_4	15252037	(A subunit or PR65); however, PP2Ac alternatively binds to alpha-4,  a subunit related to yeast Tap42 protein, which also associates with phosphatases  PP4 or PP6.	bind
46259	7	2425	6	10	NULL	0	NULL	PP6	GP		is a type of					phosphatases	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_279_37_15252037_s_4	15252037	(A subunit or PR65); however, PP2Ac alternatively binds to alpha-4,  a subunit related to yeast Tap42 protein, which also associates with phosphatases  PP4 or PP6.	bind
5695	1	2425	7	10	NULL	0	NULL	PP2Ac	GP		binds		alternatively						alpha-4 subunit		NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_279_37_15252037_s_4	15252037	(A subunit or PR65); however, PP2Ac alternatively binds to alpha-4,  a subunit related to yeast Tap42 protein, which also associates with phosphatases  PP4 or PP6.	bind
5696	2	2425	7	10	NULL	0	NULL	alpha-4 subunit	GP		is related to					Tap42 protein	GP	yeast			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_279_37_15252037_s_4	15252037	(A subunit or PR65); however, PP2Ac alternatively binds to alpha-4,  a subunit related to yeast Tap42 protein, which also associates with phosphatases  PP4 or PP6.	bind
5697	3	2425	7	10	NULL	0	NULL	PP4	GP		binds								alpha-4 subunit		NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_279_37_15252037_s_4	15252037	(A subunit or PR65); however, PP2Ac alternatively binds to alpha-4,  a subunit related to yeast Tap42 protein, which also associates with phosphatases  PP4 or PP6.	bind
5698	4	2425	7	10	NULL	0	NULL	PP6	GP		binds								alpha-4 subunit		NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_279_37_15252037_s_4	15252037	(A subunit or PR65); however, PP2Ac alternatively binds to alpha-4,  a subunit related to yeast Tap42 protein, which also associates with phosphatases  PP4 or PP6.	bind
46262	5	2425	7	10	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_279_37_15252037_s_4	15252037	(A subunit or PR65); however, PP2Ac alternatively binds to alpha-4,  a subunit related to yeast Tap42 protein, which also associates with phosphatases  PP4 or PP6.	bind
46263	6	2425	7	10	NULL	0	NULL	PP4	GP		is a type of					phosphatases	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_279_37_15252037_s_4	15252037	(A subunit or PR65); however, PP2Ac alternatively binds to alpha-4,  a subunit related to yeast Tap42 protein, which also associates with phosphatases  PP4 or PP6.	bind
46264	7	2425	7	10	NULL	0	NULL	PP6	GP		is a type of					phosphatases	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_279_37_15252037_s_4	15252037	(A subunit or PR65); however, PP2Ac alternatively binds to alpha-4,  a subunit related to yeast Tap42 protein, which also associates with phosphatases  PP4 or PP6.	bind
5444	1	2426	6	10	NULL	0	NULL	PP2Ac	GP		bind		alternatively			alpha-4	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_37_38912_s_4	15252037	(A subunit or PR65); however, PP2Ac alternatively binds to alpha-4, a subunit related to yeast Tap42 protein, which also associates with phosphatases PP4 or PP6.	bind
5445	2	2426	6	10	NULL	0	NULL	alpha-4 subunit	GP		is related to					Tap42 protein	GP	yeast			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_37_38912_s_4	15252037	(A subunit or PR65); however, PP2Ac alternatively binds to alpha-4, a subunit related to yeast Tap42 protein, which also associates with phosphatases PP4 or PP6.	bind
5446	3	2426	6	10	NULL	0	NULL	Tap42 protein	GP	yeast	associate					PP4	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_37_38912_s_4	15252037	(A subunit or PR65); however, PP2Ac alternatively binds to alpha-4, a subunit related to yeast Tap42 protein, which also associates with phosphatases PP4 or PP6.	bind
5447	4	2426	6	10	NULL	0	NULL	Tap42 protein	GP	yeast	associate					PP6	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_37_38912_s_4	15252037	(A subunit or PR65); however, PP2Ac alternatively binds to alpha-4, a subunit related to yeast Tap42 protein, which also associates with phosphatases PP4 or PP6.	bind
5448	5	2426	6	10	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_37_38912_s_4	15252037	(A subunit or PR65); however, PP2Ac alternatively binds to alpha-4, a subunit related to yeast Tap42 protein, which also associates with phosphatases PP4 or PP6.	bind
61107	6	2426	6	10	NULL	0	NULL	PP4	GP		is a type of					phosphatase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_37_38912_s_4	15252037	(A subunit or PR65); however, PP2Ac alternatively binds to alpha-4, a subunit related to yeast Tap42 protein, which also associates with phosphatases PP4 or PP6.	bind
61108	7	2426	6	10	NULL	0	NULL	PP6	GP		is a type of					phosphatase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_37_38912_s_4	15252037	(A subunit or PR65); however, PP2Ac alternatively binds to alpha-4, a subunit related to yeast Tap42 protein, which also associates with phosphatases PP4 or PP6.	bind
5449	1	2427	6	10	NULL	0	NULL	MEF2 isoforms	GP		bind					Cabin1	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5440_790_s_31	10531067	(A through D), we suspected that all isoforms of MEF2 could bind to Cabin1, as was subsequently confirmed ( 15).	bind
5699	1	2427	7	10	NULL	0	NULL	MEF2 isoforms	GP		bind					Cabin1	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5440_790_s_31	10531067	(A through D), we suspected that all isoforms of MEF2 could bind to Cabin1, as was subsequently confirmed ( 15).	bind
5601	1	2428	6	10	NULL	0	NULL	ATP	Chemical		is formed from					ADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_1_88_s_145	7788886	(A through D, top) showing formation of ATP from ADP and phosphoenolpyruvate (PEP) by sarcoplasmic reticulum (SR) - bound pyruvate kinase (PK), detected by high-performance liquid chromatography of supernatant (bottom).	bind
5602	3	2428	6	10	NULL	0	NULL	PEP	GP		is					phosphoenolpyruvate	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_1_88_s_145	7788886	(A through D, top) showing formation of ATP from ADP and phosphoenolpyruvate (PEP) by sarcoplasmic reticulum (SR) - bound pyruvate kinase (PK), detected by high-performance liquid chromatography of supernatant (bottom).	bind
5603	5	2428	6	10	NULL	0	NULL	statement 1	Process		is formed by					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_1_88_s_145	7788886	(A through D, top) showing formation of ATP from ADP and phosphoenolpyruvate (PEP) by sarcoplasmic reticulum (SR) - bound pyruvate kinase (PK), detected by high-performance liquid chromatography of supernatant (bottom).	bind
5604	7	2428	6	10	NULL	0	NULL	SR	CellComponent		is					sarcoplasmic reticulum	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_1_88_s_145	7788886	(A through D, top) showing formation of ATP from ADP and phosphoenolpyruvate (PEP) by sarcoplasmic reticulum (SR) - bound pyruvate kinase (PK), detected by high-performance liquid chromatography of supernatant (bottom).	bind
5605	8	2428	6	10	NULL	0	NULL	PK	GP		is					Pyruvate kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_1_88_s_145	7788886	(A through D, top) showing formation of ATP from ADP and phosphoenolpyruvate (PEP) by sarcoplasmic reticulum (SR) - bound pyruvate kinase (PK), detected by high-performance liquid chromatography of supernatant (bottom).	bind
46314	4	2428	6	10	NULL	0	NULL	PK	GP		bind					SR	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_1_88_s_145	7788886	(A through D, top) showing formation of ATP from ADP and phosphoenolpyruvate (PEP) by sarcoplasmic reticulum (SR) - bound pyruvate kinase (PK), detected by high-performance liquid chromatography of supernatant (bottom).	bind
61109	2	2428	6	10	NULL	0	NULL	ATP	Chemical		is formed from					PEP	GP				NULL		0	NULL	NULL	NULL	gw60_circulationres_77_1_88_s_145	7788886	(A through D, top) showing formation of ATP from ADP and phosphoenolpyruvate (PEP) by sarcoplasmic reticulum (SR) - bound pyruvate kinase (PK), detected by high-performance liquid chromatography of supernatant (bottom).	bind
61110	6	2428	6	10	NULL	0	NULL	statement 2	Process		is formed by					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_circulationres_77_1_88_s_145	7788886	(A through D, top) showing formation of ATP from ADP and phosphoenolpyruvate (PEP) by sarcoplasmic reticulum (SR) - bound pyruvate kinase (PK), detected by high-performance liquid chromatography of supernatant (bottom).	bind
61112	9	2428	6	10	NULL	0	NULL	statement 1	Process		occurs along with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_circulationres_77_1_88_s_145	7788886	(A through D, top) showing formation of ATP from ADP and phosphoenolpyruvate (PEP) by sarcoplasmic reticulum (SR) - bound pyruvate kinase (PK), detected by high-performance liquid chromatography of supernatant (bottom).	bind
5700	1	2428	7	10	NULL	0	NULL	ATP	Chemical		is formed from					ADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_1_88_s_145	7788886	(A through D, top) showing formation of ATP from ADP and phosphoenolpyruvate (PEP) by sarcoplasmic reticulum (SR) - bound pyruvate kinase (PK), detected by high-performance liquid chromatography of supernatant (bottom).	bind
5701	2	2428	7	10	NULL	0	NULL	ATP	Chemical		is formed from					PEP	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_1_88_s_145	7788886	(A through D, top) showing formation of ATP from ADP and phosphoenolpyruvate (PEP) by sarcoplasmic reticulum (SR) - bound pyruvate kinase (PK), detected by high-performance liquid chromatography of supernatant (bottom).	bind
5702	4	2428	7	10	NULL	0	NULL	statement 1	Process		is formed by					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_1_88_s_145	7788886	(A through D, top) showing formation of ATP from ADP and phosphoenolpyruvate (PEP) by sarcoplasmic reticulum (SR) - bound pyruvate kinase (PK), detected by high-performance liquid chromatography of supernatant (bottom).	bind
5703	5	2428	7	10	NULL	0	NULL	PEP	GP		is					phosphoenolpyruvate	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_1_88_s_145	7788886	(A through D, top) showing formation of ATP from ADP and phosphoenolpyruvate (PEP) by sarcoplasmic reticulum (SR) - bound pyruvate kinase (PK), detected by high-performance liquid chromatography of supernatant (bottom).	bind
5704	6	2428	7	10	NULL	0	NULL	SR	CellComponent		is					sarcoplasmic reticulum	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_1_88_s_145	7788886	(A through D, top) showing formation of ATP from ADP and phosphoenolpyruvate (PEP) by sarcoplasmic reticulum (SR) - bound pyruvate kinase (PK), detected by high-performance liquid chromatography of supernatant (bottom).	bind
5705	7	2428	7	10	NULL	0	NULL	PK	GP		is					pyruvate kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_1_88_s_145	7788886	(A through D, top) showing formation of ATP from ADP and phosphoenolpyruvate (PEP) by sarcoplasmic reticulum (SR) - bound pyruvate kinase (PK), detected by high-performance liquid chromatography of supernatant (bottom).	bind
46313	3	2428	7	10	NULL	0	NULL	PK	GP		bind					SR	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_1_88_s_145	7788886	(A through D, top) showing formation of ATP from ADP and phosphoenolpyruvate (PEP) by sarcoplasmic reticulum (SR) - bound pyruvate kinase (PK), detected by high-performance liquid chromatography of supernatant (bottom).	bind
61111	8	2428	7	10	NULL	0	NULL	statement 2	Process		is formed by					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_circulationres_77_1_88_s_145	7788886	(A through D, top) showing formation of ATP from ADP and phosphoenolpyruvate (PEP) by sarcoplasmic reticulum (SR) - bound pyruvate kinase (PK), detected by high-performance liquid chromatography of supernatant (bottom).	bind
61113	9	2428	7	10	NULL	0	NULL	statement 1	Process		occurs along with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_circulationres_77_1_88_s_145	7788886	(A through D, top) showing formation of ATP from ADP and phosphoenolpyruvate (PEP) by sarcoplasmic reticulum (SR) - bound pyruvate kinase (PK), detected by high-performance liquid chromatography of supernatant (bottom).	bind
5455	1	2429	6	10	NULL	0	NULL	FecI	GP		bind					beta''	GP		1-313		NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_6_1796_s_149	12618442	(A to C) Binding of FecI to beta''1-313	bind
5706	1	2429	7	10	NULL	0	NULL	FecI	GP		binds					beta''	GP		1-313		NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_6_1796_s_149	12618442	(A to C) Binding of FecI to beta''1-313	bind
5457	1	2431	6	10	NULL	0	NULL	p107	GP		bind					GST-cyclin A-cdk2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5380_s_316	9710622	(A to C) Western blot analysis carried out after GST precipitation of GST-cyclin A-cdk2 shows the capacity of peptides p107S and p107N, but not p107N-mut, to compete the binding of p107 to cyclin A-cdk2.	bind
5459	2	2431	6	10	NULL	0	NULL	peptide p107S	GP		bind					GST-cyclin A-cdk2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5380_s_316	9710622	(A to C) Western blot analysis carried out after GST precipitation of GST-cyclin A-cdk2 shows the capacity of peptides p107S and p107N, but not p107N-mut, to compete the binding of p107 to cyclin A-cdk2.	bind
5460	3	2431	6	10	NULL	0	NULL	statement 2	Process		competes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5380_s_316	9710622	(A to C) Western blot analysis carried out after GST precipitation of GST-cyclin A-cdk2 shows the capacity of peptides p107S and p107N, but not p107N-mut, to compete the binding of p107 to cyclin A-cdk2.	bind
5461	4	2431	6	10	NULL	0	NULL	peptide p107N	GP		bind					GST-cyclin A-cdk2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5380_s_316	9710622	(A to C) Western blot analysis carried out after GST precipitation of GST-cyclin A-cdk2 shows the capacity of peptides p107S and p107N, but not p107N-mut, to compete the binding of p107 to cyclin A-cdk2.	bind
5462	5	2431	6	10	NULL	0	NULL	statement 4	Process		competes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5380_s_316	9710622	(A to C) Western blot analysis carried out after GST precipitation of GST-cyclin A-cdk2 shows the capacity of peptides p107S and p107N, but not p107N-mut, to compete the binding of p107 to cyclin A-cdk2.	bind
5463	6	2431	6	10	NULL	0	NULL	p107N-mut	GP		does not bind					GST-cyclin A-cdk2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5380_s_316	9710622	(A to C) Western blot analysis carried out after GST precipitation of GST-cyclin A-cdk2 shows the capacity of peptides p107S and p107N, but not p107N-mut, to compete the binding of p107 to cyclin A-cdk2.	bind
5707	1	2431	7	10	NULL	0	NULL	p107 peptide	GP		binds to					GST-cyclin A-cdk2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5380_s_316	9710622	(A to C) Western blot analysis carried out after GST precipitation of GST-cyclin A-cdk2 shows the capacity of peptides p107S and p107N, but not p107N-mut, to compete the binding of p107 to cyclin A-cdk2.	bind
5708	2	2431	7	10	NULL	0	NULL	p107S peptide	GP		binds to					GST-cyclin A-cdk2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5380_s_316	9710622	(A to C) Western blot analysis carried out after GST precipitation of GST-cyclin A-cdk2 shows the capacity of peptides p107S and p107N, but not p107N-mut, to compete the binding of p107 to cyclin A-cdk2.	bind
5709	3	2431	7	10	NULL	0	NULL	p107N peptide	GP		binds to					GST-cyclin A-cdk2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5380_s_316	9710622	(A to C) Western blot analysis carried out after GST precipitation of GST-cyclin A-cdk2 shows the capacity of peptides p107S and p107N, but not p107N-mut, to compete the binding of p107 to cyclin A-cdk2.	bind
5710	4	2431	7	10	NULL	0	NULL	p107N-mut peptide	GP		does not bind					GST-cyclin A-cdk2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5380_s_316	9710622	(A to C) Western blot analysis carried out after GST precipitation of GST-cyclin A-cdk2 shows the capacity of peptides p107S and p107N, but not p107N-mut, to compete the binding of p107 to cyclin A-cdk2.	bind
5711	5	2431	7	10	NULL	0	NULL	statement 2	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5380_s_316	9710622	(A to C) Western blot analysis carried out after GST precipitation of GST-cyclin A-cdk2 shows the capacity of peptides p107S and p107N, but not p107N-mut, to compete the binding of p107 to cyclin A-cdk2.	bind
5712	6	2431	7	10	NULL	0	NULL	statement 3	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5380_s_316	9710622	(A to C) Western blot analysis carried out after GST precipitation of GST-cyclin A-cdk2 shows the capacity of peptides p107S and p107N, but not p107N-mut, to compete the binding of p107 to cyclin A-cdk2.	bind
5477	1	2432	6	10	NULL	0	NULL	MEF2	GP		bind					GLUT4	GP			MEF2 element	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_15_5143_s_340	12861002	(A to C), whereas MEF2 comprises the binding complex formed  at the GLUT4 and MCK MEF2 elements, and this binding decreases when using MOV-P nuclear  extract (D and E).	bind
5478	2	2432	6	10	NULL	0	NULL	MEF2	GP		bind					MCK 	GP			MEF2 element	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_15_5143_s_340	12861002	(A to C), whereas MEF2 comprises the binding complex formed  at the GLUT4 and MCK MEF2 elements, and this binding decreases when using MOV-P nuclear  extract (D and E).	bind
5480	3	2432	6	10	NULL	0	NULL	MOV-P nuclear extract			decreases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_15_5143_s_340	12861002	(A to C), whereas MEF2 comprises the binding complex formed  at the GLUT4 and MCK MEF2 elements, and this binding decreases when using MOV-P nuclear  extract (D and E).	bind
5481	4	2432	6	10	NULL	0	NULL	MOV-P nuclear extract			decreases					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_15_5143_s_340	12861002	(A to C), whereas MEF2 comprises the binding complex formed  at the GLUT4 and MCK MEF2 elements, and this binding decreases when using MOV-P nuclear  extract (D and E).	bind
6266	1	2432	7	10	NULL	0	NULL	MEF2	GP		binds					GLUT4	GP			MEF2 elements	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_15_5143_s_340	12861002	(A to C), whereas MEF2 comprises the binding complex formed  at the GLUT4 and MCK MEF2 elements, and this binding decreases when using MOV-P nuclear  extract (D and E).	bind
6268	2	2432	7	10	NULL	0	NULL	MEF2	GP		binds					MCK	GP			MEF2 elements	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_15_5143_s_340	12861002	(A to C), whereas MEF2 comprises the binding complex formed  at the GLUT4 and MCK MEF2 elements, and this binding decreases when using MOV-P nuclear  extract (D and E).	bind
6309	3	2432	7	10	NULL	0	NULL	MOV-P nuclear extract			decreases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_15_5143_s_340	12861002	(A to C), whereas MEF2 comprises the binding complex formed  at the GLUT4 and MCK MEF2 elements, and this binding decreases when using MOV-P nuclear  extract (D and E).	bind
6310	4	2432	7	10	NULL	0	NULL	MOV-P nuclear extract			decreases					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_15_5143_s_340	12861002	(A to C), whereas MEF2 comprises the binding complex formed  at the GLUT4 and MCK MEF2 elements, and this binding decreases when using MOV-P nuclear  extract (D and E).	bind
5482	1	2434	6	10	NULL	0	NULL	PCL	GP		bind					Ubx	GP			PRE	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_23_9_3352_s_235	12697833	(A to F) Binding of PCL, SU(Z)12, and RPD3 to the  Ubx PRE in vivo.	bind
5483	2	2434	6	10	NULL	0	NULL	SU(Z)12	GP		bind					Ubx	GP			PRE	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_23_9_3352_s_235	12697833	(A to F) Binding of PCL, SU(Z)12, and RPD3 to the  Ubx PRE in vivo.	bind
5485	3	2434	6	10	NULL	0	NULL	RPD3	GP		bind					Ubx	GP			PRE	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_23_9_3352_s_235	12697833	(A to F) Binding of PCL, SU(Z)12, and RPD3 to the  Ubx PRE in vivo.	bind
5713	1	2434	7	10	NULL	0	NULL	PCL	GP		binds					Ubx	GP			PRE	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_23_9_3352_s_235	12697833	(A to F) Binding of PCL, SU(Z)12, and RPD3 to the  Ubx PRE in vivo.	bind
5714	2	2434	7	10	NULL	0	NULL	SU(Z)12	GP		binds					Ubx	GP			PRE	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_23_9_3352_s_235	12697833	(A to F) Binding of PCL, SU(Z)12, and RPD3 to the  Ubx PRE in vivo.	bind
5715	3	2434	7	10	NULL	0	NULL	RPD3	GP		binds					Ubx	GP			PRE	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_23_9_3352_s_235	12697833	(A to F) Binding of PCL, SU(Z)12, and RPD3 to the  Ubx PRE in vivo.	bind
5487	1	2436	6	10	NULL	0	NULL	Pax6	GP		bind					glucagon	GP	mouse		G1 element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4702_s_210	12052878	(A to T in the human sequence) was chosen because it had been shown to specifically reduce Pax6 binding to the mouse glucagon G1 element ( 2).	bind
5489	2	2436	6	10	NULL	0	NULL	A to T sequence	Chemical	human	reduces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4702_s_210	12052878	(A to T in the human sequence) was chosen because it had been shown to specifically reduce Pax6 binding to the mouse glucagon G1 element ( 2).	bind
5716	1	2436	7	10	NULL	0	NULL	Pax6	GP		binds to					glucagon	GP	mouse		G1 element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4702_s_210	12052878	(A to T in the human sequence) was chosen because it had been shown to specifically reduce Pax6 binding to the mouse glucagon G1 element ( 2).	bind
46315	2	2436	7	10	NULL	0	NULL	A to T sequence	Chemical	human	reduces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4702_s_210	12052878	(A to T in the human sequence) was chosen because it had been shown to specifically reduce Pax6 binding to the mouse glucagon G1 element ( 2).	bind
5490	1	2438	6	10	NULL	0	NULL	Ac transposase	GP		bind					chromatid	Chromosome			fAc 3''-end	NULL		NULL	NULL	NULL	NULL	gw70_genetics_171_1_333_s_283	15965263	(A)  Ac transposase binds to a  fAc 3''-end and an  Ac 5''-end in the same chromatid.	bind
5491	2	2438	6	10	NULL	0	NULL	Ac transposase	GP		bind					chromatid	Chromosome			Ac 5''-end	NULL		NULL	NULL	NULL	NULL	gw70_genetics_171_1_333_s_283	15965263	(A)  Ac transposase binds to a  fAc 3''-end and an  Ac 5''-end in the same chromatid.	bind
5717	1	2438	7	10	NULL	0	NULL	Ac transposase	GP		binds					chromatid	Chromosome			fAc 3''-end	NULL		NULL	NULL	NULL	NULL	gw70_genetics_171_1_333_s_283	15965263	(A)  Ac transposase binds to a  fAc 3''-end and an  Ac 5''-end in the same chromatid.	bind
5718	2	2438	7	10	NULL	0	NULL	Ac transposase	GP		binds					chromatid	Chromosome			Ac 5''-end	NULL		NULL	NULL	NULL	NULL	gw70_genetics_171_1_333_s_283	15965263	(A)  Ac transposase binds to a  fAc 3''-end and an  Ac 5''-end in the same chromatid.	bind
5492	1	2440	6	10	NULL	0	NULL	Keap1	GP		bind					Neh2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_8_2887_s_268	16581765	(A)  Binding model of Keap1 and Neh2.	bind
6257	1	2440	7	10	NULL	0	NULL	Keap1	GP		binds					Neh2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_8_2887_s_268	16581765	(A)  Binding model of Keap1 and Neh2.	bind
5495	1	2441	6	10	NULL	0	NULL	PTF1 complexes	GP	reconstituted;;authentic	bind					Ela1	GP	wild type		PTF1 binding site	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_117_s_118	16354684	(A)  Binding of reconstituted and authentic PTF1 complexes to wild-type and mutant  Ela1 PTF1 binding sites; (B) reconstituted and authentic PTF1 bind to PTF1 binding sites  from the promoter regions of several digestive enzyme genes.	bind
5496	2	2441	6	10	NULL	0	NULL	PTF1 complexes	GP	reconstituted;;authentic	bind					Ela1	GP	mutant		PTF1 binding site	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_117_s_118	16354684	(A)  Binding of reconstituted and authentic PTF1 complexes to wild-type and mutant  Ela1 PTF1 binding sites; (B) reconstituted and authentic PTF1 bind to PTF1 binding sites  from the promoter regions of several digestive enzyme genes.	bind
5504	3	2441	6	10	NULL	0	NULL	PTF1	GP	reconstituted;;authentic	bind					digestive enzyme genes	GP			PTF1 binding site of promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_117_s_118	16354684	(A)  Binding of reconstituted and authentic PTF1 complexes to wild-type and mutant  Ela1 PTF1 binding sites; (B) reconstituted and authentic PTF1 bind to PTF1 binding sites  from the promoter regions of several digestive enzyme genes.	bind
5719	1	2441	7	10	NULL	0	NULL	PTF1 complex	GP	reconstituted;;authentic	bind					Ela1	GP	wild-type		PTF1 binding sites	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_117_s_118	16354684	(A)  Binding of reconstituted and authentic PTF1 complexes to wild-type and mutant  Ela1 PTF1 binding sites; (B) reconstituted and authentic PTF1 bind to PTF1 binding sites  from the promoter regions of several digestive enzyme genes.	bind
5720	2	2441	7	10	NULL	0	NULL	PTF1 complex	GP	reconstituted;;authentic	binds to					Ela1	GP	mutant		PTF1 binding sites	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_117_s_118	16354684	(A)  Binding of reconstituted and authentic PTF1 complexes to wild-type and mutant  Ela1 PTF1 binding sites; (B) reconstituted and authentic PTF1 bind to PTF1 binding sites  from the promoter regions of several digestive enzyme genes.	bind
5721	3	2441	7	10	NULL	0	NULL	PTF1	GP	reconstituted;;authentic	binds to					digestive enzyme	GP			PTF1 binding sites in the promoter of	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_117_s_118	16354684	(A)  Binding of reconstituted and authentic PTF1 complexes to wild-type and mutant  Ela1 PTF1 binding sites; (B) reconstituted and authentic PTF1 bind to PTF1 binding sites  from the promoter regions of several digestive enzyme genes.	bind
5506	1	2442	6	10	NULL	0	NULL			purified;;recombinant	bind			TRAP A-domain		HepG2 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_9_5883_s_157	16113307	(A)  Binding of various concentrations of the purified recombinant TRAP A-domain and GST  (as a control) to 1 x 106 HepG2 cells.	bind
5507	2	2442	6	10	NULL	0	NULL	GST	Chemical		bind					HepG2 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_9_5883_s_157	16113307	(A)  Binding of various concentrations of the purified recombinant TRAP A-domain and GST  (as a control) to 1 x 106 HepG2 cells.	bind
5722	1	2442	7	10	NULL	0	NULL			purified;;recombinant	binds to			TRAP A-domain		HepG2 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_9_5883_s_157	16113307	(A)  Binding of various concentrations of the purified recombinant TRAP A-domain and GST  (as a control) to 1 x 106 HepG2 cells.	bind
5723	2	2442	7	10	NULL	0	NULL	GST	Chemical		binds to					HepG2 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_9_5883_s_157	16113307	(A)  Binding of various concentrations of the purified recombinant TRAP A-domain and GST  (as a control) to 1 x 106 HepG2 cells.	bind
5516	1	2449	6	10	NULL	0	NULL	Importin 13	GP		bind		specifically			zz-NF-YBGST-NF-YC complex	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5339_s_275	15964792	(A)  Importin 13 was bound specifically to the immobilized zz-NF-YBGST-NF-YC complex,  and this binding was abolished by a 10-fold molar excess of NF-YA.	bind
5518	2	2449	6	10	NULL	0	NULL	NF-YA	GP	excess of	abolishes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5339_s_275	15964792	(A)  Importin 13 was bound specifically to the immobilized zz-NF-YBGST-NF-YC complex,  and this binding was abolished by a 10-fold molar excess of NF-YA.	bind
5727	1	2449	7	10	NULL	0	NULL	Importin 13	GP		binds to		specifically			 zz-NF-YBGST-NF-YC complex	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5339_s_275	15964792	(A)  Importin 13 was bound specifically to the immobilized zz-NF-YBGST-NF-YC complex,  and this binding was abolished by a 10-fold molar excess of NF-YA.	bind
5728	2	2449	7	10	NULL	0	NULL	statement 1	Process		is abolished by					NF-YA	GP	excess of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5339_s_275	15964792	(A)  Importin 13 was bound specifically to the immobilized zz-NF-YBGST-NF-YC complex,  and this binding was abolished by a 10-fold molar excess of NF-YA.	bind
5520	1	2450	6	10	NULL	0	NULL	2-MeS-ADP	Chemical		bind					platelets	Cell	human			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_brjpharmacol_132_1_47_s_139	11156560	(A)  In vitro effect of R-99224 (10 muM) combined with ARL-66096 (0.3 muM) on [3]-2-MeS-ADP binding to washed human platelets; (B)  In vitro effects of A3P5PS (300 muM) combined with R-99224 (10 muM) or ARL-66096 (0.3 muM) on [3]-2-MeS-ADP binding to washed human platelets.	bind
5733	1	2450	7	10	NULL	0	NULL	2-MeS-ADP	Chemical		bind					platelets	Cell	human			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_brjpharmacol_132_1_47_s_139	11156560	(A)  In vitro effect of R-99224 (10 muM) combined with ARL-66096 (0.3 muM) on [3]-2-MeS-ADP binding to washed human platelets; (B)  In vitro effects of A3P5PS (300 muM) combined with R-99224 (10 muM) or ARL-66096 (0.3 muM) on [3]-2-MeS-ADP binding to washed human platelets.	bind
5523	1	2451	6	10	NULL	0	NULL	MKP5	GP		bind					JNK	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8619_s_246	16166642	(a)  JAMP outcompetes MKP5 binding to JNK in vivo.	bind
5525	2	2451	6	10	NULL	0	NULL	JAMP	GP		bind					JNK	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8619_s_246	16166642	(a)  JAMP outcompetes MKP5 binding to JNK in vivo.	bind
5526	3	2451	6	10	NULL	0	NULL	statement 1	Process		outcompetes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8619_s_246	16166642	(a)  JAMP outcompetes MKP5 binding to JNK in vivo.	bind
5872	1	2451	7	10	NULL	0	NULL	MKP5	GP		binds to					JNK	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8619_s_246	16166642	(a)  JAMP outcompetes MKP5 binding to JNK in vivo.	bind
5873	2	2451	7	10	NULL	0	NULL	 JAMP	GP		bind					JNK	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8619_s_246	16166642	(a)  JAMP outcompetes MKP5 binding to JNK in vivo.	bind
7882	3	2451	7	10	NULL	0	NULL	statement 2	Process		outcompetes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8619_s_246	16166642	(a)  JAMP outcompetes MKP5 binding to JNK in vivo.	bind
5536	1	2452	6	10	NULL	0	NULL	AnaO23A5	GP		bind					A. marginale protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_12_7257_s_120	15557651	(A)  Phase-contrast microscopy was used to locate intraerythrocytic  A. marginale and the associated inclusion appendage; (B) rhodamine-phalloidin was used to label  F-actin; and (C) goat-anti-mouse IgG conjugated to Alexa 488 was used to detect MAb  AnaO23A5 bound to the  A. marginale protein.	bind
46316	2	2452	6	10	NULL	0	NULL	AnaO23A5	GP		is a type of					MAb	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_12_7257_s_120	15557651	(A)  Phase-contrast microscopy was used to locate intraerythrocytic  A. marginale and the associated inclusion appendage; (B) rhodamine-phalloidin was used to label  F-actin; and (C) goat-anti-mouse IgG conjugated to Alexa 488 was used to detect MAb  AnaO23A5 bound to the  A. marginale protein.	bind
5874	1	2452	7	10	NULL	0	NULL	AnaO23A5	GP		binds to					 A. marginale protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_12_7257_s_120	15557651	(A)  Phase-contrast microscopy was used to locate intraerythrocytic  A. marginale and the associated inclusion appendage; (B) rhodamine-phalloidin was used to label  F-actin; and (C) goat-anti-mouse IgG conjugated to Alexa 488 was used to detect MAb  AnaO23A5 bound to the  A. marginale protein.	bind
46317	2	2452	7	10	NULL	0	NULL	AnaO23A5	GP		is a type of					MAb	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_12_7257_s_120	15557651	(A)  Phase-contrast microscopy was used to locate intraerythrocytic  A. marginale and the associated inclusion appendage; (B) rhodamine-phalloidin was used to label  F-actin; and (C) goat-anti-mouse IgG conjugated to Alexa 488 was used to detect MAb  AnaO23A5 bound to the  A. marginale protein.	bind
5538	1	2453	6	10	NULL	0	NULL	Bim	GP		bind					Bcl-w	GP				NULL	epilepsy brain samples	NULL	NULL	NULL	NULL	gw70_jclininvest_113_7_1059_s_266	15057313	(A)  Representative Western blot (WB) showing Bim binding to Bcl-w immunoprecipitates  in epilepsy but not control brain samples.	bind
5539	2	2453	6	10	NULL	0	NULL	Bim	GP		does not bind					Bcl-w	GP				NULL	control brain samples	NULL	NULL	NULL	NULL	gw70_jclininvest_113_7_1059_s_266	15057313	(A)  Representative Western blot (WB) showing Bim binding to Bcl-w immunoprecipitates  in epilepsy but not control brain samples.	bind
5875	1	2453	7	10	NULL	0	NULL	Bim	GP		binds to					Bcl-w	GP				NULL	epilepsy brain sample	NULL	NULL	NULL	NULL	gw70_jclininvest_113_7_1059_s_266	15057313	(A)  Representative Western blot (WB) showing Bim binding to Bcl-w immunoprecipitates  in epilepsy but not control brain samples.	bind
61114	2	2453	7	10	NULL	0	NULL	Bim	GP		does not bind					Bcl-w	GP				NULL	control brain samples	0	NULL	NULL	NULL	gw70_jclininvest_113_7_1059_s_266	15057313	(A)  Representative Western blot (WB) showing Bim binding to Bcl-w immunoprecipitates  in epilepsy but not control brain samples.	bind
5549	1	2454	6	10	NULL	0	NULL	nuclear protein	GP		bind									C1 region	NULL	human endometrial cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_10_5795_s_219	8621448	(A)  RNA of the RL95-2 cells with a concatenated FP1 sequence in order to  isolate the nuclear protein that binds to the C1 region in human  endometrial cells.	bind
5876	1	2454	7	10	NULL	0	NULL	nuclear protein	GP		binds									C1 region	NULL	human endometrial cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_10_5795_s_219	8621448	(A)  RNA of the RL95-2 cells with a concatenated FP1 sequence in order to  isolate the nuclear protein that binds to the C1 region in human  endometrial cells.	bind
5550	1	2455	6	10	NULL	0	NULL	MSL	GP		bind		weakly			X chromosome	Chromosome				NULL	roX1 roX2 double mutant male nucleus	NULL	NULL	NULL	NULL	gw60_molcell_11_4_977_s_199	12718883	(A)  roX1 roX2 double mutant male nucleus showing weak MSL binding to the X chromosome and ectopic binding to autosomal sites and heterochromatin (arrowhead).	bind
5551	2	2455	6	10	NULL	0	NULL	MSL	GP		bind		ectopicaly			autosomal sites	Chromosome				NULL	roX1 roX2 double mutant male nucleus	NULL	NULL	NULL	NULL	gw60_molcell_11_4_977_s_199	12718883	(A)  roX1 roX2 double mutant male nucleus showing weak MSL binding to the X chromosome and ectopic binding to autosomal sites and heterochromatin (arrowhead).	bind
5552	3	2455	6	10	NULL	0	NULL	MSL	GP		bind		ectopicaly			heterochromatin	Chromosome				NULL	roX1 roX2 double mutant male nucleus	NULL	NULL	NULL	NULL	gw60_molcell_11_4_977_s_199	12718883	(A)  roX1 roX2 double mutant male nucleus showing weak MSL binding to the X chromosome and ectopic binding to autosomal sites and heterochromatin (arrowhead).	bind
5877	1	2455	7	10	NULL	0	NULL	MSL	GP		binds		weakly			X chromosome	Chromosome				NULL	roX1 roX2 double mutant male nucleus	NULL	NULL	NULL	NULL	gw60_molcell_11_4_977_s_199	12718883	(A)  roX1 roX2 double mutant male nucleus showing weak MSL binding to the X chromosome and ectopic binding to autosomal sites and heterochromatin (arrowhead).	bind
5878	2	2455	7	10	NULL	0	NULL	MSL	GP		binds		ectopically			autosomal sites	Chromosome				NULL	roX1 roX2 double mutant male nucleus	NULL	NULL	NULL	NULL	gw60_molcell_11_4_977_s_199	12718883	(A)  roX1 roX2 double mutant male nucleus showing weak MSL binding to the X chromosome and ectopic binding to autosomal sites and heterochromatin (arrowhead).	bind
5879	3	2455	7	10	NULL	0	NULL	MSL	GP		binds		ectopically			heterochromatin	Chromosome				NULL	roX1 roX2 double mutant male nucleus	NULL	NULL	NULL	NULL	gw60_molcell_11_4_977_s_199	12718883	(A)  roX1 roX2 double mutant male nucleus showing weak MSL binding to the X chromosome and ectopic binding to autosomal sites and heterochromatin (arrowhead).	bind
5554	1	2457	6	10	NULL	0	NULL	MeCP2	GP		bind					Uqcrc1	GP			promoter	NULL	wild type mouse brain	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_13_5033_s_193	16782889	(a)  Uqcrc1 promoter map showing CpG frequency, methylation status, and the region used for PCR  amplification of immunoprecipitated DNA. (b) Chromatin immunoprecipitation reveals  MeCP2 bound to the  Uqcrc1 promoter in wt mouse brain but not in  Mecp2-null mouse brain.	bind
5555	2	2457	6	10	NULL	0	NULL	MeCP2	GP		does not bind					Uqcrc1	GP			promoter	NULL	Mecp2-null mouse brain	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_13_5033_s_193	16782889	(a)  Uqcrc1 promoter map showing CpG frequency, methylation status, and the region used for PCR  amplification of immunoprecipitated DNA. (b) Chromatin immunoprecipitation reveals  MeCP2 bound to the  Uqcrc1 promoter in wt mouse brain but not in  Mecp2-null mouse brain.	bind
5880	1	2457	7	10	NULL	0	NULL	MeCP2	GP		binds					Uqcrc1	GP			promoter	NULL	wt mouse brain	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_13_5033_s_193	16782889	(a)  Uqcrc1 promoter map showing CpG frequency, methylation status, and the region used for PCR  amplification of immunoprecipitated DNA. (b) Chromatin immunoprecipitation reveals  MeCP2 bound to the  Uqcrc1 promoter in wt mouse brain but not in  Mecp2-null mouse brain.	bind
5881	2	2457	7	10	NULL	0	NULL	MeCP2	GP		does not bind					Uqcrc1	GP			promoter	NULL	Mecp2-null mouse brain	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_13_5033_s_193	16782889	(a)  Uqcrc1 promoter map showing CpG frequency, methylation status, and the region used for PCR  amplification of immunoprecipitated DNA. (b) Chromatin immunoprecipitation reveals  MeCP2 bound to the  Uqcrc1 promoter in wt mouse brain but not in  Mecp2-null mouse brain.	bind
5562	1	2459	6	10	NULL	0	NULL	PAX6	GP		bind			PD		hGC 	GP			1BL sequence	NULL		NULL	NULL	NULL	NULL	gw60_gene_245_2_319_s_88	10717483	(A) ( Epstein et al., 1994), but not by the Pax-6 HD binding sequence P3 (   Czerny et al., 1997) (  Fig. 2A), suggesting that PAX6 bound the hGC 1BL sequence through its PD.	bind
5885	1	2459	7	10	NULL	0	NULL	PAX6 	GP		binds			 PD		hGC	GP			1BL sequence	NULL		NULL	NULL	NULL	NULL	gw60_gene_245_2_319_s_88	10717483	(A) ( Epstein et al., 1994), but not by the Pax-6 HD binding sequence P3 (   Czerny et al., 1997) (  Fig. 2A), suggesting that PAX6 bound the hGC 1BL sequence through its PD.	bind
5563	1	2460	6	10	NULL	0	NULL	melittin	GP		bind					POPC vesicles	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_1_26_s_204	15533303	(A) (a) Kinetics of the helix formation upon melittin binding to POPC vesicles  (Ri=90; [POPC]=3 mM; [melittin]=35  M).	bind
5886	1	2460	7	10	NULL	0	NULL	melittin	GP		binds					POPC vesicles	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_1_26_s_204	15533303	(A) (a) Kinetics of the helix formation upon melittin binding to POPC vesicles  (Ri=90; [POPC]=3 mM; [melittin]=35  M).	bind
5564	1	2462	6	10	NULL	0	NULL	THC	GP		bind					SMC	GP				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_120_2_91_s_161	14741398	(A) (lane 4) and poly (U) (lane 6) displaced THC  binding to the SMC, while poly (C) displaced neither SMC nor FMC.	bind
5566	3	2462	6	10	NULL	0	NULL	statement 2	Process		displaces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_120_2_91_s_161	14741398	(A) (lane 4) and poly (U) (lane 6) displaced THC  binding to the SMC, while poly (C) displaced neither SMC nor FMC.	bind
5569	4	2462	6	10	NULL	0	NULL	poly (C)	Chemical		does not displace					SMC	GP				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_120_2_91_s_161	14741398	(A) (lane 4) and poly (U) (lane 6) displaced THC  binding to the SMC, while poly (C) displaced neither SMC nor FMC.	bind
5571	5	2462	6	10	NULL	0	NULL	poly (C)	Chemical		does not displace					FMC	GP				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_120_2_91_s_161	14741398	(A) (lane 4) and poly (U) (lane 6) displaced THC  binding to the SMC, while poly (C) displaced neither SMC nor FMC.	bind
46318	2	2462	6	10	NULL	0	NULL	poly (U) 	Chemical		bind					SMC	GP				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_120_2_91_s_161	14741398	(A) (lane 4) and poly (U) (lane 6) displaced THC  binding to the SMC, while poly (C) displaced neither SMC nor FMC.	bind
5887	1	2462	7	10	NULL	0	NULL	THC	GP		binds					SMC	GP				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_120_2_91_s_161	14741398	(A) (lane 4) and poly (U) (lane 6) displaced THC  binding to the SMC, while poly (C) displaced neither SMC nor FMC.	bind
5888	2	2462	7	10	NULL	0	NULL	poly (U)	Chemical		binds					SMC	GP				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_120_2_91_s_161	14741398	(A) (lane 4) and poly (U) (lane 6) displaced THC  binding to the SMC, while poly (C) displaced neither SMC nor FMC.	bind
5889	3	2462	7	10	NULL	0	NULL	poly (U)	Chemical		displaces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_120_2_91_s_161	14741398	(A) (lane 4) and poly (U) (lane 6) displaced THC  binding to the SMC, while poly (C) displaced neither SMC nor FMC.	bind
5890	4	2462	7	10	NULL	0	NULL	poly (C)	Chemical		does not displace					SMC	GP				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_120_2_91_s_161	14741398	(A) (lane 4) and poly (U) (lane 6) displaced THC  binding to the SMC, while poly (C) displaced neither SMC nor FMC.	bind
5891	5	2462	7	10	NULL	0	NULL	poly (C)	Chemical		does not displace					FMC	GP				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_120_2_91_s_161	14741398	(A) (lane 4) and poly (U) (lane 6) displaced THC  binding to the SMC, while poly (C) displaced neither SMC nor FMC.	bind
5572	1	2465	6	10	NULL	0	NULL	RIM1	GP		bind					Munc13	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_30_1_183_s_112	11343654	(A) (Left) RIM1 binding to Munc13 GST fusion proteins in cosedimentation assays.	bind
46319	2	2465	6	10	NULL	0	NULL	Munc13	GP		is a type of					GST fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_30_1_183_s_112	11343654	(A) (Left) RIM1 binding to Munc13 GST fusion proteins in cosedimentation assays.	bind
5892	1	2465	7	10	NULL	0	NULL	RIM1	GP		binds					Munc13	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_30_1_183_s_112	11343654	(A) (Left) RIM1 binding to Munc13 GST fusion proteins in cosedimentation assays.	bind
46320	2	2465	7	10	NULL	0	NULL	Munc13	GP		is a type of					GST fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_30_1_183_s_112	11343654	(A) (Left) RIM1 binding to Munc13 GST fusion proteins in cosedimentation assays.	bind
5573	1	2467	6	NULL	NULL	0	NULL	PP2A A subunit protein	NULL		bind	NULL				Hsc-70	NULL				NULL	bovine liver cytosol	0	NULL	NULL	NULL	gw60_cellbiol_160_5_699_s_151	12604586	(A) 100 mug of GST or GST fusion peptide corresponding to the PP2A A subunit protein was bound to glutathione-Sepharose beads and used to pull down Hsc-70 from 2 mg of bovine liver cytosol.	bind
46321	2	2467	6	10	NULL	0	NULL	PP2A A subunit protein	NULL		is a type of	NULL				GST fusion peptide	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_160_5_699_s_151	12604586	(A) 100 mug of GST or GST fusion peptide corresponding to the PP2A A subunit protein was bound to glutathione-Sepharose beads and used to pull down Hsc-70 from 2 mg of bovine liver cytosol.	bind
5973	1	2467	7	10	NULL	0	NULL	PP2A A subunit protein 	NULL		binds	NULL				Hsc-70	NULL				NULL	bovine liver cytosol	NULL	NULL	NULL	NULL	gw60_cellbiol_160_5_699_s_151	12604586	(A) 100 mug of GST or GST fusion peptide corresponding to the PP2A A subunit protein was bound to glutathione-Sepharose beads and used to pull down Hsc-70 from 2 mg of bovine liver cytosol.	bind
46322	2	2467	7	10	NULL	0	NULL	PP2A A subunit protein	NULL		is a type of	NULL				GST fusion peptide	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_160_5_699_s_151	12604586	(A) 100 mug of GST or GST fusion peptide corresponding to the PP2A A subunit protein was bound to glutathione-Sepharose beads and used to pull down Hsc-70 from 2 mg of bovine liver cytosol.	bind
5574	1	2468	6	10	NULL	0	NULL	lactoferrin	GP	125I-labeled;;recombinant;;human	bind		specifically			Kupffer cells	Cell	mouse			NULL		NULL	NULL	NULL	NULL	gw60_clindiagnlabimmun_8_6_1234_s_134	11687469	(a) 125I-labeled recombinant human lactoferrin specifically bound to mouse Kupffer cells.	bind
5893	1	2468	7	10	NULL	0	NULL	 lactoferrin	GP	125I-labeled;;recombinant;;human	binds		specifically			Kupffer cells	Cell	mouse			NULL		NULL	NULL	NULL	NULL	gw60_clindiagnlabimmun_8_6_1234_s_134	11687469	(a) 125I-labeled recombinant human lactoferrin specifically bound to mouse Kupffer cells.	bind
5575	1	2469	6	10	NULL	0	NULL	293T cells	Cell		express		transiently			Hck499F	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_18_6984_s_112	10958693	(A) 293T cells transiently expressing Hck499F or  tsHck499F were incubated at the indicated temperature for 48 h and then lysed with NP-40 lysis buffer.	bind
5576	2	2469	6	10	NULL	0	NULL	293T cells	Cell		express		transiently			tsHck499F	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_18_6984_s_112	10958693	(A) 293T cells transiently expressing Hck499F or  tsHck499F were incubated at the indicated temperature for 48 h and then lysed with NP-40 lysis buffer.	bind
6557	1	2469	7	10	NULL	0	NULL	 293T cells	Cell		express		transiently			Hck499F	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_18_6984_s_112	10958693	(A) 293T cells transiently expressing Hck499F or  tsHck499F were incubated at the indicated temperature for 48 h and then lysed with NP-40 lysis buffer.	bind
6558	2	2469	7	10	NULL	0	NULL	293T cells	Cell		express		transiently			tsHck499F	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_18_6984_s_112	10958693	(A) 293T cells transiently expressing Hck499F or  tsHck499F were incubated at the indicated temperature for 48 h and then lysed with NP-40 lysis buffer.	bind
5577	1	2471	6	10	NULL	0	NULL	HIRA	GP	35S-labeled	bind					GST-H2B	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5546_s_187	9710638	(A) 35S-labeled HIRA binds GST-H2B and GST-HIRIP3 but not GST immobilized on glutathione beads.	bind
5578	2	2471	6	10	NULL	0	NULL	HIRA	GP	35S-labeled	bind					GST-HIRIP3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5546_s_187	9710638	(A) 35S-labeled HIRA binds GST-H2B and GST-HIRIP3 but not GST immobilized on glutathione beads.	bind
5579	3	2471	6	10	NULL	0	NULL	HIRA	GP	35S-labeled	does not bind					GST	Chemical	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5546_s_187	9710638	(A) 35S-labeled HIRA binds GST-H2B and GST-HIRIP3 but not GST immobilized on glutathione beads.	bind
5895	1	2471	7	10	NULL	0	NULL	HIRA	GP	35S-labeled	binds					GST-H2B	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5546_s_187	9710638	(A) 35S-labeled HIRA binds GST-H2B and GST-HIRIP3 but not GST immobilized on glutathione beads.	bind
5896	2	2471	7	10	NULL	0	NULL	HIRA	GP	35S-labeled	binds					GST-HIRIP3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5546_s_187	9710638	(A) 35S-labeled HIRA binds GST-H2B and GST-HIRIP3 but not GST immobilized on glutathione beads.	bind
5897	3	2471	7	10	NULL	0	NULL	HIRA	GP	35S-labeled	does not bind					GST	Chemical	immobilized 			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5546_s_187	9710638	(A) 35S-labeled HIRA binds GST-H2B and GST-HIRIP3 but not GST immobilized on glutathione beads.	bind
5580	1	2473	6	10	NULL	0	NULL	prohibitin	GP	35S-labeled	bind					GST-Phb	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_312_2_459_s_92	14637159	(A) 35S-labeled prohibitin binds to GST-Phb but not control GST beads in vitro.	bind
5581	2	2473	6	10	NULL	0	NULL	prohibitin	GP	35S-labeled	does not bind					GST	Chemical	control			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_312_2_459_s_92	14637159	(A) 35S-labeled prohibitin binds to GST-Phb but not control GST beads in vitro.	bind
5898	1	2473	7	10	NULL	0	NULL	prohibitin	GP	35S-labeled	binds					GST-Phb	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_312_2_459_s_92	14637159	(A) 35S-labeled prohibitin binds to GST-Phb but not control GST beads in vitro.	bind
5899	2	2473	7	10	NULL	0	NULL	prohibitin	GP	35S-labeled	does not bind					GST	Chemical	control			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_312_2_459_s_92	14637159	(A) 35S-labeled prohibitin binds to GST-Phb but not control GST beads in vitro.	bind
5582	1	2474	6	10	NULL	0	NULL	SGP1	GP		bind					c-erbB-3	GP		extracellular epitope		NULL	untreated MCF-7 fractions	NULL	NULL	NULL	NULL	gw60_cellbiol_157_6_929_s_87	12045181	(A) 400 mug protein from untreated (-) or LMB-treated (+) C or N MCF-7 fractions were immunoprecipitated (IP) with SGP1, which detects an extracellular epitope of c-erbB-3, or with mIgG1 and blotted (IB) with C17, which binds to the cytoplasmic part of c-erbB-3.	bind
5583	2	2474	6	10	NULL	0	NULL	SGP1	GP		bind					c-erbB-3	GP		extracellular epitope		NULL	LMB-treated (+) MCF-7 fractions	NULL	NULL	NULL	NULL	gw60_cellbiol_157_6_929_s_87	12045181	(A) 400 mug protein from untreated (-) or LMB-treated (+) C or N MCF-7 fractions were immunoprecipitated (IP) with SGP1, which detects an extracellular epitope of c-erbB-3, or with mIgG1 and blotted (IB) with C17, which binds to the cytoplasmic part of c-erbB-3.	bind
5584	3	2474	6	10	NULL	0	NULL	C17	GP		bind					c-erbB-3	GP		cytoplasmic part		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_6_929_s_87	12045181	(A) 400 mug protein from untreated (-) or LMB-treated (+) C or N MCF-7 fractions were immunoprecipitated (IP) with SGP1, which detects an extracellular epitope of c-erbB-3, or with mIgG1 and blotted (IB) with C17, which binds to the cytoplasmic part of c-erbB-3.	bind
6330	1	2474	7	10	NULL	0	NULL	SGP1	GP		binds					c-erbB-3 \t	GP		extracellular epitope		NULL	untreated MCF-7 fractions	NULL	NULL	NULL	NULL	gw60_cellbiol_157_6_929_s_87	12045181	(A) 400 mug protein from untreated (-) or LMB-treated (+) C or N MCF-7 fractions were immunoprecipitated (IP) with SGP1, which detects an extracellular epitope of c-erbB-3, or with mIgG1 and blotted (IB) with C17, which binds to the cytoplasmic part of c-erbB-3.	bind
6331	2	2474	7	10	NULL	0	NULL	SGP1	GP		bind					c-erbB-3	GP		extracellular epitope		NULL	LMB-treated (+) MCF-7 fractions	NULL	NULL	NULL	NULL	gw60_cellbiol_157_6_929_s_87	12045181	(A) 400 mug protein from untreated (-) or LMB-treated (+) C or N MCF-7 fractions were immunoprecipitated (IP) with SGP1, which detects an extracellular epitope of c-erbB-3, or with mIgG1 and blotted (IB) with C17, which binds to the cytoplasmic part of c-erbB-3.	bind
6334	3	2474	7	10	NULL	0	NULL	C17	GP		binds					c-erbB-3	GP		cytoplasmic part		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_6_929_s_87	12045181	(A) 400 mug protein from untreated (-) or LMB-treated (+) C or N MCF-7 fractions were immunoprecipitated (IP) with SGP1, which detects an extracellular epitope of c-erbB-3, or with mIgG1 and blotted (IB) with C17, which binds to the cytoplasmic part of c-erbB-3.	bind
5585	1	2475	6	10	NULL	0	NULL	GTP S	Chemical		bind					5-ht5A/HEK293 membranes	CellComponent	guinea pig			NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_51_3_566_s_207	16846620	(A) 5-HT-induced stimulation of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes in the absence, and presence, of SB-699551-A (0.1, 0.3, 1 and 3   M).	bind
5586	2	2475	6	10	NULL	0	NULL	5-HT	Chemical		induced					statement 1	Process	stimulation of			NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_51_3_566_s_207	16846620	(A) 5-HT-induced stimulation of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes in the absence, and presence, of SB-699551-A (0.1, 0.3, 1 and 3   M).	bind
5906	1	2475	7	10	NULL	0	NULL	GTP S	Chemical		binds					5-ht5A/HEK293 membranes	CellComponent	guinea pig			NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_51_3_566_s_207	16846620	(A) 5-HT-induced stimulation of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes in the absence, and presence, of SB-699551-A (0.1, 0.3, 1 and 3   M).	bind
5907	2	2475	7	10	NULL	0	NULL	5-HT	Chemical		induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_51_3_566_s_207	16846620	(A) 5-HT-induced stimulation of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes in the absence, and presence, of SB-699551-A (0.1, 0.3, 1 and 3   M).	bind
5587	1	2477	6	10	NULL	0	NULL	9G8	GP		bind					Flag-TAP	GP				NULL	transfected cells	NULL	NULL	NULL	NULL	gw60_molcell_11_3_837_s_31	12667464	(A) 9G8 binds Flag-TAP in transfected cells.	bind
6335	1	2477	7	10	NULL	0	NULL	9G8	GP		binds					Flag-TAP	GP				NULL	transfected cells	NULL	NULL	NULL	NULL	gw60_molcell_11_3_837_s_31	12667464	(A) 9G8 binds Flag-TAP in transfected cells.	bind
7631	1	2478	6	10	NULL	0	NULL	cis-acting elements	NucleicAcid		involved in					fbp1	GP	regulation of transcription			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6426_s_103	10938120	(A) A deletion series was constructed within the  fbp1 promoter of the  fbp1-lacZ reporter to identify  cis-acting elements involved in the regulation of  fbp1 transcription.	bind
6336	1	2478	7	10	NULL	0	NULL	cis-acting elements	NucleicAcid		involved in 					fbp1	GP	regulation of transcription of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6426_s_103	10938120	(A) A deletion series was constructed within the  fbp1 promoter of the  fbp1-lacZ reporter to identify  cis-acting elements involved in the regulation of  fbp1 transcription.	bind
5588	1	2481	6	10	NULL	0	NULL	repressosome	GP		bind									I* element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4219_s_433	10330162	(A) A multiprotein complex (repressosome) binds to the I* element.	bind
46323	2	2481	6	10	NULL	0	NULL	repressosome	GP		is a type of					multiprotein complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4219_s_433	10330162	(A) A multiprotein complex (repressosome) binds to the I* element.	bind
6337	1	2481	7	10	NULL	0	NULL	repressosome	GP		binds									I* element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4219_s_433	10330162	(A) A multiprotein complex (repressosome) binds to the I* element.	bind
46324	2	2481	7	10	NULL	0	NULL	repressosome	GP		is a type of					multiprotein complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4219_s_433	10330162	(A) A multiprotein complex (repressosome) binds to the I* element.	bind
5589	1	2483	6	10	NULL	0	NULL	PKN	GP		bind			effector domain		RhoA	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_4_5_793_s_53	10619026	(A) A ribbon representation of the PKN effector domain (blue) bound to RhoA (brown).	bind
6339	1	2483	7	10	NULL	0	NULL	 PKN	GP		binds			effector domain		RhoA	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_4_5_793_s_53	10619026	(A) A ribbon representation of the PKN effector domain (blue) bound to RhoA (brown).	bind
5590	1	2484	6	10	NULL	0	NULL	eIF4A	GP		bind					eIF4G	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_1_26_s_365	12482958	(A) A sandwich model of eIF4A binding to eIF4G is shown ( 32).	bind
6340	1	2484	7	10	NULL	0	NULL	eIF4A	GP		binds					eIF4G	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_1_26_s_365	12482958	(A) A sandwich model of eIF4A binding to eIF4G is shown ( 32).	bind
5591	1	2485	6	10	NULL	0	NULL	single P. aeruginosa bacterium	Organism		bind					PM 	CellComponent				NULL	CFTE cell	NULL	NULL	NULL	NULL	gw60_febslett_405_2_200_s_113	9089291	(A) A single  P. aeruginosa bacterium bound to the plasma membrane of a CFTE cell (magnification=14800x); (B) a single bacterium bound to the plasma membrane (PM) of a CFTE cell and encircled by microvilli (magnification=23040x); (C) two bacteria entrapped inside a CFTE cell within a vacuole (V) (magnification=6320x); (D) a single bacterium in contact with a mitochondrion inside a CFTE cell (magnification=6122x); (E,F) bacteria penetrating HTE cells (normal cells) forming deep invaginations (magnifications=26730x and 25740x, respectively).	bind
5592	2	2485	6	10	NULL	0	NULL	PM	CellComponent		is					plasma membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_febslett_405_2_200_s_113	9089291	(A) A single  P. aeruginosa bacterium bound to the plasma membrane of a CFTE cell (magnification=14800x); (B) a single bacterium bound to the plasma membrane (PM) of a CFTE cell and encircled by microvilli (magnification=23040x); (C) two bacteria entrapped inside a CFTE cell within a vacuole (V) (magnification=6320x); (D) a single bacterium in contact with a mitochondrion inside a CFTE cell (magnification=6122x); (E,F) bacteria penetrating HTE cells (normal cells) forming deep invaginations (magnifications=26730x and 25740x, respectively).	bind
5593	3	2485	6	10	NULL	0	NULL	statement 1	Process		encircled by					microvilli	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_febslett_405_2_200_s_113	9089291	(A) A single  P. aeruginosa bacterium bound to the plasma membrane of a CFTE cell (magnification=14800x); (B) a single bacterium bound to the plasma membrane (PM) of a CFTE cell and encircled by microvilli (magnification=23040x); (C) two bacteria entrapped inside a CFTE cell within a vacuole (V) (magnification=6320x); (D) a single bacterium in contact with a mitochondrion inside a CFTE cell (magnification=6122x); (E,F) bacteria penetrating HTE cells (normal cells) forming deep invaginations (magnifications=26730x and 25740x, respectively).	bind
5594	4	2485	6	10	NULL	0	NULL	P. aeruginosa bacteria	Organism		entrapped inside					vacuole	CellComponent				NULL	CFTE cell	NULL	NULL	NULL	NULL	gw60_febslett_405_2_200_s_113	9089291	(A) A single  P. aeruginosa bacterium bound to the plasma membrane of a CFTE cell (magnification=14800x); (B) a single bacterium bound to the plasma membrane (PM) of a CFTE cell and encircled by microvilli (magnification=23040x); (C) two bacteria entrapped inside a CFTE cell within a vacuole (V) (magnification=6320x); (D) a single bacterium in contact with a mitochondrion inside a CFTE cell (magnification=6122x); (E,F) bacteria penetrating HTE cells (normal cells) forming deep invaginations (magnifications=26730x and 25740x, respectively).	bind
5595	5	2485	6	10	NULL	0	NULL	P. aeruginosa bacteria	Organism		is in contact with					mitochondria	CellComponent				NULL	CFTE cell	NULL	NULL	NULL	NULL	gw60_febslett_405_2_200_s_113	9089291	(A) A single  P. aeruginosa bacterium bound to the plasma membrane of a CFTE cell (magnification=14800x); (B) a single bacterium bound to the plasma membrane (PM) of a CFTE cell and encircled by microvilli (magnification=23040x); (C) two bacteria entrapped inside a CFTE cell within a vacuole (V) (magnification=6320x); (D) a single bacterium in contact with a mitochondrion inside a CFTE cell (magnification=6122x); (E,F) bacteria penetrating HTE cells (normal cells) forming deep invaginations (magnifications=26730x and 25740x, respectively).	bind
5596	6	2485	6	10	NULL	0	NULL	P. aeruginosa bacteria	Organism		penetrate					HTE cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_febslett_405_2_200_s_113	9089291	(A) A single  P. aeruginosa bacterium bound to the plasma membrane of a CFTE cell (magnification=14800x); (B) a single bacterium bound to the plasma membrane (PM) of a CFTE cell and encircled by microvilli (magnification=23040x); (C) two bacteria entrapped inside a CFTE cell within a vacuole (V) (magnification=6320x); (D) a single bacterium in contact with a mitochondrion inside a CFTE cell (magnification=6122x); (E,F) bacteria penetrating HTE cells (normal cells) forming deep invaginations (magnifications=26730x and 25740x, respectively).	bind
5597	7	2485	6	10	NULL	0	NULL	statement 6	Process		form					invaginations	Process	deep			NULL		NULL	NULL	NULL	NULL	gw60_febslett_405_2_200_s_113	9089291	(A) A single  P. aeruginosa bacterium bound to the plasma membrane of a CFTE cell (magnification=14800x); (B) a single bacterium bound to the plasma membrane (PM) of a CFTE cell and encircled by microvilli (magnification=23040x); (C) two bacteria entrapped inside a CFTE cell within a vacuole (V) (magnification=6320x); (D) a single bacterium in contact with a mitochondrion inside a CFTE cell (magnification=6122x); (E,F) bacteria penetrating HTE cells (normal cells) forming deep invaginations (magnifications=26730x and 25740x, respectively).	bind
6341	1	2485	7	10	NULL	0	NULL	P. aeruginosa bacterium	Organism		binds to					plasma membrane	CellComponent				NULL	CFTE cell	NULL	NULL	NULL	NULL	gw60_febslett_405_2_200_s_113	9089291	(A) A single  P. aeruginosa bacterium bound to the plasma membrane of a CFTE cell (magnification=14800x); (B) a single bacterium bound to the plasma membrane (PM) of a CFTE cell and encircled by microvilli (magnification=23040x); (C) two bacteria entrapped inside a CFTE cell within a vacuole (V) (magnification=6320x); (D) a single bacterium in contact with a mitochondrion inside a CFTE cell (magnification=6122x); (E,F) bacteria penetrating HTE cells (normal cells) forming deep invaginations (magnifications=26730x and 25740x, respectively).	bind
6342	2	2485	7	10	NULL	0	NULL	statement 1	Process		is encircled by					microvilli	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_febslett_405_2_200_s_113	9089291	(A) A single  P. aeruginosa bacterium bound to the plasma membrane of a CFTE cell (magnification=14800x); (B) a single bacterium bound to the plasma membrane (PM) of a CFTE cell and encircled by microvilli (magnification=23040x); (C) two bacteria entrapped inside a CFTE cell within a vacuole (V) (magnification=6320x); (D) a single bacterium in contact with a mitochondrion inside a CFTE cell (magnification=6122x); (E,F) bacteria penetrating HTE cells (normal cells) forming deep invaginations (magnifications=26730x and 25740x, respectively).	bind
6343	3	2485	7	10	NULL	0	NULL	bacteria	Organism		trapped inside					vacuole	CellComponent				NULL	CFTE cell	NULL	NULL	NULL	NULL	gw60_febslett_405_2_200_s_113	9089291	(A) A single  P. aeruginosa bacterium bound to the plasma membrane of a CFTE cell (magnification=14800x); (B) a single bacterium bound to the plasma membrane (PM) of a CFTE cell and encircled by microvilli (magnification=23040x); (C) two bacteria entrapped inside a CFTE cell within a vacuole (V) (magnification=6320x); (D) a single bacterium in contact with a mitochondrion inside a CFTE cell (magnification=6122x); (E,F) bacteria penetrating HTE cells (normal cells) forming deep invaginations (magnifications=26730x and 25740x, respectively).	bind
6344	4	2485	7	10	NULL	0	NULL	bacterium	Organism		is in contact with					mitochondria	CellComponent				NULL	CFTE cell	NULL	NULL	NULL	NULL	gw60_febslett_405_2_200_s_113	9089291	(A) A single  P. aeruginosa bacterium bound to the plasma membrane of a CFTE cell (magnification=14800x); (B) a single bacterium bound to the plasma membrane (PM) of a CFTE cell and encircled by microvilli (magnification=23040x); (C) two bacteria entrapped inside a CFTE cell within a vacuole (V) (magnification=6320x); (D) a single bacterium in contact with a mitochondrion inside a CFTE cell (magnification=6122x); (E,F) bacteria penetrating HTE cells (normal cells) forming deep invaginations (magnifications=26730x and 25740x, respectively).	bind
6345	5	2485	7	10	NULL	0	NULL	bacteria	Organism		penetrates					HTE cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_febslett_405_2_200_s_113	9089291	(A) A single  P. aeruginosa bacterium bound to the plasma membrane of a CFTE cell (magnification=14800x); (B) a single bacterium bound to the plasma membrane (PM) of a CFTE cell and encircled by microvilli (magnification=23040x); (C) two bacteria entrapped inside a CFTE cell within a vacuole (V) (magnification=6320x); (D) a single bacterium in contact with a mitochondrion inside a CFTE cell (magnification=6122x); (E,F) bacteria penetrating HTE cells (normal cells) forming deep invaginations (magnifications=26730x and 25740x, respectively).	bind
6346	6	2485	7	10	NULL	0	NULL	statement 5	Process		forms					invaginations	Process	deep			NULL		NULL	NULL	NULL	NULL	gw60_febslett_405_2_200_s_113	9089291	(A) A single  P. aeruginosa bacterium bound to the plasma membrane of a CFTE cell (magnification=14800x); (B) a single bacterium bound to the plasma membrane (PM) of a CFTE cell and encircled by microvilli (magnification=23040x); (C) two bacteria entrapped inside a CFTE cell within a vacuole (V) (magnification=6320x); (D) a single bacterium in contact with a mitochondrion inside a CFTE cell (magnification=6122x); (E,F) bacteria penetrating HTE cells (normal cells) forming deep invaginations (magnifications=26730x and 25740x, respectively).	bind
6347	7	2485	7	10	NULL	0	NULL	PM	CellComponent		is					plasma membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_febslett_405_2_200_s_113	9089291	(A) A single  P. aeruginosa bacterium bound to the plasma membrane of a CFTE cell (magnification=14800x); (B) a single bacterium bound to the plasma membrane (PM) of a CFTE cell and encircled by microvilli (magnification=23040x); (C) two bacteria entrapped inside a CFTE cell within a vacuole (V) (magnification=6320x); (D) a single bacterium in contact with a mitochondrion inside a CFTE cell (magnification=6122x); (E,F) bacteria penetrating HTE cells (normal cells) forming deep invaginations (magnifications=26730x and 25740x, respectively).	bind
6348	8	2485	7	10	NULL	0	NULL	V	CellComponent		is					Vacuole	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_febslett_405_2_200_s_113	9089291	(A) A single  P. aeruginosa bacterium bound to the plasma membrane of a CFTE cell (magnification=14800x); (B) a single bacterium bound to the plasma membrane (PM) of a CFTE cell and encircled by microvilli (magnification=23040x); (C) two bacteria entrapped inside a CFTE cell within a vacuole (V) (magnification=6320x); (D) a single bacterium in contact with a mitochondrion inside a CFTE cell (magnification=6122x); (E,F) bacteria penetrating HTE cells (normal cells) forming deep invaginations (magnifications=26730x and 25740x, respectively).	bind
5598	1	2486	6	10	NULL	0	NULL	HRP-2	GP		bind					heme	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_9_8_881_s_98	12204687	(A) a strong inhibitor, compound  24, and (B) a weak inhibitor,  10, on heme binding by HRP-2 using the microtiterplate assay described under Experimental Procedures.	bind
5599	2	2486	6	10	NULL	0	NULL	compound 24	Chemical		inhibits		strongly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_9_8_881_s_98	12204687	(A) a strong inhibitor, compound  24, and (B) a weak inhibitor,  10, on heme binding by HRP-2 using the microtiterplate assay described under Experimental Procedures.	bind
5600	3	2486	6	10	NULL	0	NULL	compound 10	Chemical		inhibits		weakly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_9_8_881_s_98	12204687	(A) a strong inhibitor, compound  24, and (B) a weak inhibitor,  10, on heme binding by HRP-2 using the microtiterplate assay described under Experimental Procedures.	bind
6349	1	2486	7	10	NULL	0	NULL	heme	Chemical		binds					HRP-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_9_8_881_s_98	12204687	(A) a strong inhibitor, compound  24, and (B) a weak inhibitor,  10, on heme binding by HRP-2 using the microtiterplate assay described under Experimental Procedures.	bind
6350	2	2486	7	10	NULL	0	NULL	compound 24	Chemical		inhibit		strongly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_9_8_881_s_98	12204687	(A) a strong inhibitor, compound  24, and (B) a weak inhibitor,  10, on heme binding by HRP-2 using the microtiterplate assay described under Experimental Procedures.	bind
6351	3	2486	7	10	NULL	0	NULL	compound 10	Chemical		inhibit		weakly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_9_8_881_s_98	12204687	(A) a strong inhibitor, compound  24, and (B) a weak inhibitor,  10, on heme binding by HRP-2 using the microtiterplate assay described under Experimental Procedures.	bind
5617	1	2487	6	10	NULL	0	NULL	CREB	GP		bind			DNA binding domain 		DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_967_s_155	9447994	(A) A-CREB, but not A-VBP or A-Fos, inhibits the DNA binding activity of the DNA binding domain of CREB.	bind
5618	2	2487	6	10	NULL	0	NULL	A-CREB	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_967_s_155	9447994	(A) A-CREB, but not A-VBP or A-Fos, inhibits the DNA binding activity of the DNA binding domain of CREB.	bind
5619	3	2487	6	10	NULL	0	NULL	A-VBP	GP		does not inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_967_s_155	9447994	(A) A-CREB, but not A-VBP or A-Fos, inhibits the DNA binding activity of the DNA binding domain of CREB.	bind
5622	4	2487	6	10	NULL	0	NULL	A-Fos	GP		does not inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_967_s_155	9447994	(A) A-CREB, but not A-VBP or A-Fos, inhibits the DNA binding activity of the DNA binding domain of CREB.	bind
5624	5	2487	6	10	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_967_s_155	9447994	(A) A-CREB, but not A-VBP or A-Fos, inhibits the DNA binding activity of the DNA binding domain of CREB.	bind
6352	1	2487	7	10	NULL	0	NULL	CREB	GP		binds			DNA binding domain		DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_967_s_155	9447994	(A) A-CREB, but not A-VBP or A-Fos, inhibits the DNA binding activity of the DNA binding domain of CREB.	bind
6353	2	2487	7	10	NULL	0	NULL	A-CREB	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_967_s_155	9447994	(A) A-CREB, but not A-VBP or A-Fos, inhibits the DNA binding activity of the DNA binding domain of CREB.	bind
6354	3	2487	7	10	NULL	0	NULL	A-VBP	GP		does not inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_967_s_155	9447994	(A) A-CREB, but not A-VBP or A-Fos, inhibits the DNA binding activity of the DNA binding domain of CREB.	bind
6355	4	2487	7	10	NULL	0	NULL	A-Fos	GP		does not inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_967_s_155	9447994	(A) A-CREB, but not A-VBP or A-Fos, inhibits the DNA binding activity of the DNA binding domain of CREB.	bind
61116	5	2487	7	10	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_2_967_s_155	9447994	(A) A-CREB, but not A-VBP or A-Fos, inhibits the DNA binding activity of the DNA binding domain of CREB.	bind
5628	1	2488	6	10	NULL	0	NULL	A190	GP		bind		stably			Net1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_1_45_s_126	11511359	(A) A190 but not Nop1 binds stably to Net1.	bind
5629	2	2488	6	10	NULL	0	NULL	Nop1	GP		does not bind					Net1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_1_45_s_126	11511359	(A) A190 but not Nop1 binds stably to Net1.	bind
6356	1	2488	7	10	NULL	0	NULL	A190	GP		binds 		stably			Net1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_1_45_s_126	11511359	(A) A190 but not Nop1 binds stably to Net1.	bind
6357	2	2488	7	10	NULL	0	NULL	Nop1	GP		does not bind					Net1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_1_45_s_126	11511359	(A) A190 but not Nop1 binds stably to Net1.	bind
5633	1	2490	6	10	NULL	0	NULL	GTP	Chemical		bind					Ras	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_7_386_s_50	9545198	(a) Accumulation of the GTP-bound form of Ras (Ras-GTP) as a function of time.	bind
6361	1	2490	7	10	NULL	0	NULL	GTP	Chemical		binds					Ras	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_7_386_s_50	9545198	(a) Accumulation of the GTP-bound form of Ras (Ras-GTP) as a function of time.	bind
5634	1	2491	6	10	NULL	0	NULL	CBP	GP		acetylates					GCMa 	GP		TAD		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8401_s_332	16166624	(A) Acetylation of GCMa TAD by CBP increases  its transcriptional activity and protein stability.	bind
5635	2	2491	6	10	NULL	0	NULL	statement 1	Process		increases					GCMa	GP	transcriptional activity of	TAD		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8401_s_332	16166624	(A) Acetylation of GCMa TAD by CBP increases  its transcriptional activity and protein stability.	bind
5636	3	2491	6	10	NULL	0	NULL	statement 1	Process		increases					GCMa	GP	protein stability of	TAD		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8401_s_332	16166624	(A) Acetylation of GCMa TAD by CBP increases  its transcriptional activity and protein stability.	bind
6362	1	2491	7	10	NULL	0	NULL	CBP	GP		acetylates					GCMa 	GP		TAD		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8401_s_332	16166624	(A) Acetylation of GCMa TAD by CBP increases  its transcriptional activity and protein stability.	bind
6363	2	2491	7	10	NULL	0	NULL	statement 1	Process		increases					GCMa	GP	transcriptional activity of	TAD		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8401_s_332	16166624	(A) Acetylation of GCMa TAD by CBP increases  its transcriptional activity and protein stability.	bind
6364	3	2491	7	10	NULL	0	NULL	statement 1	Process		increases					GCMa	GP	protein stability of	TAD		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8401_s_332	16166624	(A) Acetylation of GCMa TAD by CBP increases  its transcriptional activity and protein stability.	bind
5637	1	2493	6	10	NULL	0	NULL	ARF1	GP	activated	bind		selectively			SNARE	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_2_281_s_34	15657398	(A) Activated ARF1 binds selectively to SNARE cargo proteins.	bind
46325	2	2493	6	10	NULL	0	NULL	SNARE	GP		is a type of					cargo proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_2_281_s_34	15657398	(A) Activated ARF1 binds selectively to SNARE cargo proteins.	bind
6365	1	2493	7	10	NULL	0	NULL	ARF1	GP	activated	binds to		selectively			SNARE	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_2_281_s_34	15657398	(A) Activated ARF1 binds selectively to SNARE cargo proteins.	bind
46326	2	2493	7	10	NULL	0	NULL	SNARE	GP		is a type of					cargo proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_2_281_s_34	15657398	(A) Activated ARF1 binds selectively to SNARE cargo proteins.	bind
5729	1	2494	6	10	NULL	0	NULL	Ly49H NK cell receptor	GP		bind					MCMV m157 gene product	GP				NULL	C57BL/6 mouse strain	NULL	NULL	NULL	NULL	gw70_microbesinfect_5_13_1263_s_119	14623023	(A) Activation of NK cells in C57BL/6 mouse strain is a consequence of binding  of the Ly49H NK cell receptor to the MCMV  m157 gene product, leading to efficacious virus control in vivo, which can be compromised  by depletion of NK cells.	bind
5730	2	2494	6	10	NULL	0	NULL	NK cells	Cell	activation of	is a consequence of 					statement 1	Process				NULL	C57BL/6 mouse strain	NULL	NULL	NULL	NULL	gw70_microbesinfect_5_13_1263_s_119	14623023	(A) Activation of NK cells in C57BL/6 mouse strain is a consequence of binding  of the Ly49H NK cell receptor to the MCMV  m157 gene product, leading to efficacious virus control in vivo, which can be compromised  by depletion of NK cells.	bind
5731	3	2494	6	10	NULL	0	NULL	statement 1	Process		leads to					virus control	Process	efficacious			NULL	in vivo	NULL	NULL	NULL	NULL	gw70_microbesinfect_5_13_1263_s_119	14623023	(A) Activation of NK cells in C57BL/6 mouse strain is a consequence of binding  of the Ly49H NK cell receptor to the MCMV  m157 gene product, leading to efficacious virus control in vivo, which can be compromised  by depletion of NK cells.	bind
5732	4	2494	6	10	NULL	0	NULL	NK cells	Cell	depletion of 	compromises					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_microbesinfect_5_13_1263_s_119	14623023	(A) Activation of NK cells in C57BL/6 mouse strain is a consequence of binding  of the Ly49H NK cell receptor to the MCMV  m157 gene product, leading to efficacious virus control in vivo, which can be compromised  by depletion of NK cells.	bind
6366	1	2494	7	10	NULL	0	NULL	Ly49H NK cell receptor	GP		binds to					MCMV m157 gene product	GP				NULL	C57BL/6 mouse strain	NULL	NULL	NULL	NULL	gw70_microbesinfect_5_13_1263_s_119	14623023	(A) Activation of NK cells in C57BL/6 mouse strain is a consequence of binding  of the Ly49H NK cell receptor to the MCMV  m157 gene product, leading to efficacious virus control in vivo, which can be compromised  by depletion of NK cells.	bind
6367	2	2494	7	10	NULL	0	NULL	NK cells 	Cell	 activation of	is a consequence of					statement 1	Process				NULL	C57BL/6 mouse strain	NULL	NULL	NULL	NULL	gw70_microbesinfect_5_13_1263_s_119	14623023	(A) Activation of NK cells in C57BL/6 mouse strain is a consequence of binding  of the Ly49H NK cell receptor to the MCMV  m157 gene product, leading to efficacious virus control in vivo, which can be compromised  by depletion of NK cells.	bind
6368	3	2494	7	10	NULL	0	NULL	statement 1	Process		leads to					 virus control	Process	efficacious			NULL	in vivo	NULL	NULL	NULL	NULL	gw70_microbesinfect_5_13_1263_s_119	14623023	(A) Activation of NK cells in C57BL/6 mouse strain is a consequence of binding  of the Ly49H NK cell receptor to the MCMV  m157 gene product, leading to efficacious virus control in vivo, which can be compromised  by depletion of NK cells.	bind
6369	4	2494	7	10	NULL	0	NULL	statement 1	Cell		is compromised by					NK cells	Cell	depletion of			NULL		NULL	NULL	NULL	NULL	gw70_microbesinfect_5_13_1263_s_119	14623023	(A) Activation of NK cells in C57BL/6 mouse strain is a consequence of binding  of the Ly49H NK cell receptor to the MCMV  m157 gene product, leading to efficacious virus control in vivo, which can be compromised  by depletion of NK cells.	bind
5883	1	2495	6	10	NULL	0	NULL	tTA	GP		bind									TRE	NULL	293 Tet-Off cells	NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1393_s_127	11359930	(A) Activation of the transactivator tTA, a fusion protein consisting of the tet-repressor and the VP16 activation domain, by removal of doxycycline (Dox) from the culture medium results in the binding of tTA to the tet-responsive element TRE and transcription of Flag-tagged HD exon 1 fragments with 20, 51, and 83 CAG repeats in 293 Tet-Off cells.	bind
5884	2	2495	6	10	NULL	0	NULL	TRE	NucleicAcid		is					tet-responsive element	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1393_s_127	11359930	(A) Activation of the transactivator tTA, a fusion protein consisting of the tet-repressor and the VP16 activation domain, by removal of doxycycline (Dox) from the culture medium results in the binding of tTA to the tet-responsive element TRE and transcription of Flag-tagged HD exon 1 fragments with 20, 51, and 83 CAG repeats in 293 Tet-Off cells.	bind
6204	3	2495	6	10	NULL	0	NULL	tTA	GP		consists of					tet repressor	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1393_s_127	11359930	(A) Activation of the transactivator tTA, a fusion protein consisting of the tet-repressor and the VP16 activation domain, by removal of doxycycline (Dox) from the culture medium results in the binding of tTA to the tet-responsive element TRE and transcription of Flag-tagged HD exon 1 fragments with 20, 51, and 83 CAG repeats in 293 Tet-Off cells.	bind
6205	4	2495	6	10	NULL	0	NULL	tTA 	GP		is a type of					transactivator	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1393_s_127	11359930	(A) Activation of the transactivator tTA, a fusion protein consisting of the tet-repressor and the VP16 activation domain, by removal of doxycycline (Dox) from the culture medium results in the binding of tTA to the tet-responsive element TRE and transcription of Flag-tagged HD exon 1 fragments with 20, 51, and 83 CAG repeats in 293 Tet-Off cells.	bind
6206	5	2495	6	10	NULL	0	NULL	tTA	GP		consists of								VP16 activation domain		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1393_s_127	11359930	(A) Activation of the transactivator tTA, a fusion protein consisting of the tet-repressor and the VP16 activation domain, by removal of doxycycline (Dox) from the culture medium results in the binding of tTA to the tet-responsive element TRE and transcription of Flag-tagged HD exon 1 fragments with 20, 51, and 83 CAG repeats in 293 Tet-Off cells.	bind
6207	6	2495	6	10	NULL	0	NULL	doxycycline	Chemical		is removed from					culture medium	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1393_s_127	11359930	(A) Activation of the transactivator tTA, a fusion protein consisting of the tet-repressor and the VP16 activation domain, by removal of doxycycline (Dox) from the culture medium results in the binding of tTA to the tet-responsive element TRE and transcription of Flag-tagged HD exon 1 fragments with 20, 51, and 83 CAG repeats in 293 Tet-Off cells.	bind
6208	7	2495	6	10	NULL	0	NULL	statement 6	Process		results in					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1393_s_127	11359930	(A) Activation of the transactivator tTA, a fusion protein consisting of the tet-repressor and the VP16 activation domain, by removal of doxycycline (Dox) from the culture medium results in the binding of tTA to the tet-responsive element TRE and transcription of Flag-tagged HD exon 1 fragments with 20, 51, and 83 CAG repeats in 293 Tet-Off cells.	bind
6209	8	2495	6	10	NULL	0	NULL	statement 6	Process		results in					HD exon1	GP	transcription of		CAG repeats	NULL	293 Tet-Off cells	NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1393_s_127	11359930	(A) Activation of the transactivator tTA, a fusion protein consisting of the tet-repressor and the VP16 activation domain, by removal of doxycycline (Dox) from the culture medium results in the binding of tTA to the tet-responsive element TRE and transcription of Flag-tagged HD exon 1 fragments with 20, 51, and 83 CAG repeats in 293 Tet-Off cells.	bind
46327	9	2495	6	10	NULL	0	NULL	tTA	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1393_s_127	11359930	(A) Activation of the transactivator tTA, a fusion protein consisting of the tet-repressor and the VP16 activation domain, by removal of doxycycline (Dox) from the culture medium results in the binding of tTA to the tet-responsive element TRE and transcription of Flag-tagged HD exon 1 fragments with 20, 51, and 83 CAG repeats in 293 Tet-Off cells.	bind
6370	1	2495	7	10	NULL	0	NULL	tTA	GP		binds to									TRE	NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1393_s_127	11359930	(A) Activation of the transactivator tTA, a fusion protein consisting of the tet-repressor and the VP16 activation domain, by removal of doxycycline (Dox) from the culture medium results in the binding of tTA to the tet-responsive element TRE and transcription of Flag-tagged HD exon 1 fragments with 20, 51, and 83 CAG repeats in 293 Tet-Off cells.	bind
6371	2	2495	7	10	NULL	0	NULL	 tTA	GP		consist of					tet-repressor	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1393_s_127	11359930	(A) Activation of the transactivator tTA, a fusion protein consisting of the tet-repressor and the VP16 activation domain, by removal of doxycycline (Dox) from the culture medium results in the binding of tTA to the tet-responsive element TRE and transcription of Flag-tagged HD exon 1 fragments with 20, 51, and 83 CAG repeats in 293 Tet-Off cells.	bind
6372	3	2495	7	10	NULL	0	NULL	tTA	GP		consist of								VP16 activation domain		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1393_s_127	11359930	(A) Activation of the transactivator tTA, a fusion protein consisting of the tet-repressor and the VP16 activation domain, by removal of doxycycline (Dox) from the culture medium results in the binding of tTA to the tet-responsive element TRE and transcription of Flag-tagged HD exon 1 fragments with 20, 51, and 83 CAG repeats in 293 Tet-Off cells.	bind
6373	4	2495	7	10	NULL	0	NULL	tTA	GP		is a type of					transactivator	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1393_s_127	11359930	(A) Activation of the transactivator tTA, a fusion protein consisting of the tet-repressor and the VP16 activation domain, by removal of doxycycline (Dox) from the culture medium results in the binding of tTA to the tet-responsive element TRE and transcription of Flag-tagged HD exon 1 fragments with 20, 51, and 83 CAG repeats in 293 Tet-Off cells.	bind
6374	5	2495	7	10	NULL	0	NULL	tTA	GP	activation of	results in					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1393_s_127	11359930	(A) Activation of the transactivator tTA, a fusion protein consisting of the tet-repressor and the VP16 activation domain, by removal of doxycycline (Dox) from the culture medium results in the binding of tTA to the tet-responsive element TRE and transcription of Flag-tagged HD exon 1 fragments with 20, 51, and 83 CAG repeats in 293 Tet-Off cells.	bind
6375	6	2495	7	10	NULL	0	NULL	doxycycline	Chemical	 	removed from					culture medium	Chemical			CAG repeats	NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1393_s_127	11359930	(A) Activation of the transactivator tTA, a fusion protein consisting of the tet-repressor and the VP16 activation domain, by removal of doxycycline (Dox) from the culture medium results in the binding of tTA to the tet-responsive element TRE and transcription of Flag-tagged HD exon 1 fragments with 20, 51, and 83 CAG repeats in 293 Tet-Off cells.	bind
6376	7	2495	7	10	NULL	0	NULL	tTA	GP	activation of	results in					HD exon1	GP	transcription of		CAG repeats \t	NULL	293 Tet-Off cells	NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1393_s_127	11359930	(A) Activation of the transactivator tTA, a fusion protein consisting of the tet-repressor and the VP16 activation domain, by removal of doxycycline (Dox) from the culture medium results in the binding of tTA to the tet-responsive element TRE and transcription of Flag-tagged HD exon 1 fragments with 20, 51, and 83 CAG repeats in 293 Tet-Off cells.	bind
6377	8	2495	7	10	NULL	0	NULL	statement 1	Process		occurs after					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1393_s_127	11359930	(A) Activation of the transactivator tTA, a fusion protein consisting of the tet-repressor and the VP16 activation domain, by removal of doxycycline (Dox) from the culture medium results in the binding of tTA to the tet-responsive element TRE and transcription of Flag-tagged HD exon 1 fragments with 20, 51, and 83 CAG repeats in 293 Tet-Off cells.	bind
6379	10	2495	7	10	NULL	0	NULL	Dox	Chemical		is					doxycycline	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1393_s_127	11359930	(A) Activation of the transactivator tTA, a fusion protein consisting of the tet-repressor and the VP16 activation domain, by removal of doxycycline (Dox) from the culture medium results in the binding of tTA to the tet-responsive element TRE and transcription of Flag-tagged HD exon 1 fragments with 20, 51, and 83 CAG repeats in 293 Tet-Off cells.	bind
46328	9	2495	7	10	NULL	0	NULL	TRE	NucleicAcid		is					tet-responsive element	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1393_s_127	11359930	(A) Activation of the transactivator tTA, a fusion protein consisting of the tet-repressor and the VP16 activation domain, by removal of doxycycline (Dox) from the culture medium results in the binding of tTA to the tet-responsive element TRE and transcription of Flag-tagged HD exon 1 fragments with 20, 51, and 83 CAG repeats in 293 Tet-Off cells.	bind
5900	1	2497	6	10	NULL	0	NULL	uPA	GP	active	bind					uPAR	GP				NULL	PM	NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1467_s_296	11359936	(A) Active uPA binds to uPAR on the PM.	bind
6380	1	2497	7	10	NULL	0	NULL	uPA	GP	active	binds to					uPAR	GP				NULL	PM	NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1467_s_296	11359936	(A) Active uPA binds to uPAR on the PM.	bind
5901	1	2498	6	10	NULL	0	NULL	Activin	GP		bind					ActRIIB receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_93_4_557_s_198	9604931	(A) Activin  binds to ActRIIB receptors in a concentration-dependent manner.	bind
5902	2	2498	6	10	NULL	0	NULL	statement 1	GP		is dependent on					concentration	QuantityOrMeasure				NULL		NULL	NULL	NULL	NULL	gw60_cell_93_4_557_s_198	9604931	(A) Activin  binds to ActRIIB receptors in a concentration-dependent manner.	bind
6381	1	2498	7	10	NULL	0	NULL	Activin	GP		binds to					ActRIIB receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_93_4_557_s_198	9604931	(A) Activin  binds to ActRIIB receptors in a concentration-dependent manner.	bind
6382	2	2498	7	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				concentration	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cell_93_4_557_s_198	9604931	(A) Activin  binds to ActRIIB receptors in a concentration-dependent manner.	bind
5903	1	2499	6	10	NULL	0	NULL	Ad12 E1B protein	GP		bind		directly			PCAF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5540_s_294	10891493	(A) Ad12 E1B 55-kDa protein binds directly to PCAF.	bind
6383	1	2499	7	10	NULL	0	NULL	Ad12 E1B protein	GP		binds		directly			PCAF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5540_s_294	10891493	(A) Ad12 E1B 55-kDa protein binds directly to PCAF.	bind
5904	1	2500	6	10	NULL	0	NULL	CPSF	GP		bind					class I RNA	NucleicAcid			RNA element	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_52_33654_s_197	8969235	(A) addition data, the binding of CPSF to the class I RNA containing both RNA elements was greater than to the RNAs containing either element alone (Fig.  3 C, 8.1,  lane 3).	bind
6384	1	2500	7	10	NULL	0	NULL	CPSF	GP		binds					class I RNA	NucleicAcid			RNA element	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_52_33654_s_197	8969235	(A) addition data, the binding of CPSF to the class I RNA containing both RNA elements was greater than to the RNAs containing either element alone (Fig.  3 C, 8.1,  lane 3).	bind
5905	1	2502	6	10	NULL	0	NULL	V-ATPase	GP		bind			V1 domain on E subunit		H6.1 MAb	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_2_575_s_227	15632060	(a) After cell  stimulation, V-ATPase was immunoprecipitated from the lysates with H6.1 MAb, which  binds the V1 domain on its E subunit.	bind
5908	2	2502	6	10	NULL	0	NULL	statement 1	Process		occurs after					cell stimulation	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_2_575_s_227	15632060	(a) After cell  stimulation, V-ATPase was immunoprecipitated from the lysates with H6.1 MAb, which  binds the V1 domain on its E subunit.	bind
6386	1	2502	7	10	NULL	0	NULL	V-ATPase	GP		binds					H6.1 MAb	GP		V1 domain E subunit		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_2_575_s_227	15632060	(a) After cell  stimulation, V-ATPase was immunoprecipitated from the lysates with H6.1 MAb, which  binds the V1 domain on its E subunit.	bind
6387	2	2502	7	10	NULL	0	NULL	statement 1	Process		occurs after					cell stimulation	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_2_575_s_227	15632060	(a) After cell  stimulation, V-ATPase was immunoprecipitated from the lysates with H6.1 MAb, which  binds the V1 domain on its E subunit.	bind
5909	1	2503	6	10	NULL	0	NULL	Akt	GP		phosphorylate					p300	GP		Ser-1834		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_15_6592_s_272	16024795	(A) Akt phosphorylation of p300 at Ser-1834 binds p/CAF in vitro.	bind
5910	2	2503	6	10	NULL	0	NULL	statement 1	Process		bind					p/CAF	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_15_6592_s_272	16024795	(A) Akt phosphorylation of p300 at Ser-1834 binds p/CAF in vitro.	bind
6388	2	2503	7	10	NULL	0	NULL	statement 1	Process		binds					p/CAF	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_15_6592_s_272	16024795	(A) Akt phosphorylation of p300 at Ser-1834 binds p/CAF in vitro.	bind
6389	1	2503	7	10	NULL	0	NULL	Akt	GP		phosphorylates					p300	GP		Ser-1834		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_15_6592_s_272	16024795	(A) Akt phosphorylation of p300 at Ser-1834 binds p/CAF in vitro.	bind
5911	1	2505	6	10	NULL	0	NULL	transcription factor	GP	drosophila	bind			eh-1 like sequences		Gro	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_24_10711_s_80	16314497	(A) Alignment of eh1-like sequences found in  Drosophila transcription factors that bind Gro in vitro (C).	bind
6391	1	2505	7	10	NULL	0	NULL	transcription factors	GP	Drosophila	binds			eh1-like sequences		Gro	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_24_10711_s_80	16314497	(A) Alignment of eh1-like sequences found in  Drosophila transcription factors that bind Gro in vitro (C).	bind
5912	2	2507	6	10	NULL	0	NULL	statement 1	Process		bind					MAb	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_74_10_5529_s_82	16988228	(A) Alignment of the  P. yoelii YM AMA1 protein sequence with the deduced 7-mer sequences from phage clones that  bound to the MAb.	bind
46330	1	2507	6	10	NULL	0	NULL	phage clones			contains					7-mer sequences	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_74_10_5529_s_82	16988228	(A) Alignment of the  P. yoelii YM AMA1 protein sequence with the deduced 7-mer sequences from phage clones that  bound to the MAb.	bind
6464	2	2507	7	10	NULL	0	NULL	statement 1	Process		bind					MAb	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_74_10_5529_s_82	16988228	(A) Alignment of the  P. yoelii YM AMA1 protein sequence with the deduced 7-mer sequences from phage clones that  bound to the MAb.	bind
46331	1	2507	7	10	NULL	0	NULL	phage clones			contains					7-mer sequences	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_74_10_5529_s_82	16988228	(A) Alignment of the  P. yoelii YM AMA1 protein sequence with the deduced 7-mer sequences from phage clones that  bound to the MAb.	bind
5913	1	2511	6	10	NULL	0	NULL	Met4-myc	GP	endogenous	bind					MET25	GP	biotinylated		promoter	NULL	extracts prepared from cells 	NULL	NULL	NULL	NULL	gw60_cell_102_3_303_s_239	10975521	(A) All forms  of Met4 bind to the  MET25 promoter: Extracts prepared from cells expressing endogenous  Met4-myc and Cbf1-HA (PY752) were incubated with biotinylated  MET25 promotor fragments or a  biotinylated control DNA.	bind
5914	2	2511	6	10	NULL	0	NULL	Cbf1-HA	GP	endogenous	bind			PY752		MET25	GP	biotinylated		promoter	NULL	extracts prepared from cells 	NULL	NULL	NULL	NULL	gw60_cell_102_3_303_s_239	10975521	(A) All forms  of Met4 bind to the  MET25 promoter: Extracts prepared from cells expressing endogenous  Met4-myc and Cbf1-HA (PY752) were incubated with biotinylated  MET25 promotor fragments or a  biotinylated control DNA.	bind
6465	1	2511	7	10	NULL	0	NULL	Met4-myc	GP	endogenous	binds					MET25	GP	biotinylated		promoter	NULL	extracts prepared from cells 	NULL	NULL	NULL	NULL	gw60_cell_102_3_303_s_239	10975521	(A) All forms  of Met4 bind to the  MET25 promoter: Extracts prepared from cells expressing endogenous  Met4-myc and Cbf1-HA (PY752) were incubated with biotinylated  MET25 promotor fragments or a  biotinylated control DNA.	bind
46332	2	2511	7	10	NULL	0	NULL	Cbf1-HA	GP	endogenous	bind			PY752		MET25	GP	biotinylated		promoter	NULL	extracts prepared from cells 	NULL	NULL	NULL	NULL	gw60_cell_102_3_303_s_239	10975521	(A) All forms  of Met4 bind to the  MET25 promoter: Extracts prepared from cells expressing endogenous  Met4-myc and Cbf1-HA (PY752) were incubated with biotinylated  MET25 promotor fragments or a  biotinylated control DNA.	bind
5915	1	2514	6	10	NULL	0	NULL	CD14-IgG	GP		bind					cortical neurons	Cell	primary			NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_50_2_229_s_147	16289250	(A) Amounts of a CD14-IgG chimera that  bound to primary cortical neurons pre-treated with 10 ng/ml prostaglandins as shown.	bind
5916	2	2514	6	10	NULL	0	NULL	cortical neurons	Cell	primary	pre-treated with					prostaglandins	GP				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_50_2_229_s_147	16289250	(A) Amounts of a CD14-IgG chimera that  bound to primary cortical neurons pre-treated with 10 ng/ml prostaglandins as shown.	bind
46333	3	2514	6	10	NULL	0	NULL	CD14-IgG	GP		is a type of					chimera	GP				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_50_2_229_s_147	16289250	(A) Amounts of a CD14-IgG chimera that  bound to primary cortical neurons pre-treated with 10 ng/ml prostaglandins as shown.	bind
6466	1	2514	7	10	NULL	0	NULL	CD14-IgG	GP		binds to					cortical neurons	Cell	primary			NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_50_2_229_s_147	16289250	(A) Amounts of a CD14-IgG chimera that  bound to primary cortical neurons pre-treated with 10 ng/ml prostaglandins as shown.	bind
6467	2	2514	7	10	NULL	0	NULL	cortical neurons	Cell	primary	is pretreated with					prostaglandins	GP				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_50_2_229_s_147	16289250	(A) Amounts of a CD14-IgG chimera that  bound to primary cortical neurons pre-treated with 10 ng/ml prostaglandins as shown.	bind
46335	3	2514	7	10	NULL	0	NULL	CD14-IgG	GP		is a type of					chimera	GP				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_50_2_229_s_147	16289250	(A) Amounts of a CD14-IgG chimera that  bound to primary cortical neurons pre-treated with 10 ng/ml prostaglandins as shown.	bind
5917	1	2515	6	10	NULL	0	NULL	xpt RNAs	NucleicAcid	in vitro-transcribed	bind					guanine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_113_5_577_s_148	12787499	(A) An equilibrium dialysis strategy was used to confirm that in vitro-transcribed 93  xpt RNAs bind to guanine and can discriminate against various analogs.	bind
6468	1	2515	7	10	NULL	0	NULL	xpt RNA	NucleicAcid	in vitro-transcribed 	binds					guanine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_113_5_577_s_148	12787499	(A) An equilibrium dialysis strategy was used to confirm that in vitro-transcribed 93  xpt RNAs bind to guanine and can discriminate against various analogs.	bind
5919	1	2516	6	10	NULL	0	NULL	MAP2	GP		bind					microtubule	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_305_1_72_s_60	12732198	(A) An SDS-PAGE showing the  binding of MAP2 to microtubules at pH 6.9.	bind
6469	1	2516	7	10	NULL	0	NULL	MAP2	GP		binds					microtubules	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_305_1_72_s_60	12732198	(A) An SDS-PAGE showing the  binding of MAP2 to microtubules at pH 6.9.	bind
5921	1	2518	6	10	NULL	0	NULL	p150-Spir	GP		bind			four WH2 domains		actin monomer	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_6_345_s_22	10744979	(a) An unique array of structural motifs in p150-Spir: an acidic region, four WH2 domains, which bind monomeric actin, a modified FYVE Zn-Finger structure and a JNK-binding domain at the carboxyl terminus containing a DEJL motif.	bind
6470	1	2518	7	10	NULL	0	NULL	p150-Spir	GP		binds			four WH2 domains		actin monomer	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_6_345_s_22	10744979	(a) An unique array of structural motifs in p150-Spir: an acidic region, four WH2 domains, which bind monomeric actin, a modified FYVE Zn-Finger structure and a JNK-binding domain at the carboxyl terminus containing a DEJL motif.	bind
5925	1	2519	6	10	NULL	0	NULL	TAF6 protein derivatives	GP	purified	bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_1_206_s_132	15601843	(A) Analysis  of the DNA binding of purified TAF6 and TAF9 protein derivatives either alone or  as a complex by EMSA.	bind
5926	2	2519	6	10	NULL	0	NULL	TAF9 protein derivatives	GP	purified	bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_1_206_s_132	15601843	(A) Analysis  of the DNA binding of purified TAF6 and TAF9 protein derivatives either alone or  as a complex by EMSA.	bind
5927	3	2519	6	10	NULL	0	NULL	TAF6 protein derivatives	GP	purified	forms a complex with					TAF9 protein derivatives	GP	purified			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_1_206_s_132	15601843	(A) Analysis  of the DNA binding of purified TAF6 and TAF9 protein derivatives either alone or  as a complex by EMSA.	bind
7859	4	2519	6	10	NULL	0	NULL	statement 3	Process		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_1_206_s_132	15601843	(A) Analysis  of the DNA binding of purified TAF6 and TAF9 protein derivatives either alone or  as a complex by EMSA.	bind
6487	1	2519	7	10	NULL	0	NULL	TAF6 protein derivatives	GP	purified	bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_1_206_s_132	15601843	(A) Analysis  of the DNA binding of purified TAF6 and TAF9 protein derivatives either alone or  as a complex by EMSA.	bind
6490	2	2519	7	10	NULL	0	NULL	TAF9 protein derivatives	GP	purified	bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_1_206_s_132	15601843	(A) Analysis  of the DNA binding of purified TAF6 and TAF9 protein derivatives either alone or  as a complex by EMSA.	bind
6491	3	2519	7	10	NULL	0	NULL	TAF6 protein derivatives	GP	purified	forms a complex with					TAF9 protein derivatives	GP	purified			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_1_206_s_132	15601843	(A) Analysis  of the DNA binding of purified TAF6 and TAF9 protein derivatives either alone or  as a complex by EMSA.	bind
6496	4	2519	7	10	NULL	0	NULL	statement 3	Process		binds					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_1_206_s_132	15601843	(A) Analysis  of the DNA binding of purified TAF6 and TAF9 protein derivatives either alone or  as a complex by EMSA.	bind
5933	2	2520	6	10	NULL	0	NULL	MMP-8	GP	latent	bind					collagen	GP				NULL	GCF	NULL	NULL	NULL	NULL	gw60_infectimmun_67_5_2319_s_228	10225890	(A) Analysis of active and latent forms of MMP-8 from GCF that bind to collagen.	bind
5934	1	2520	6	10	NULL	0	NULL	MMP-8	GP	active	bind					collagen	GP				NULL	GCF	NULL	NULL	NULL	NULL	gw60_infectimmun_67_5_2319_s_228	10225890	(A) Analysis of active and latent forms of MMP-8 from GCF that bind to collagen.	bind
6497	1	2520	7	10	NULL	0	NULL	MMP-8	GP	active	binds					collagen	GP				NULL	GCF	NULL	NULL	NULL	NULL	gw60_infectimmun_67_5_2319_s_228	10225890	(A) Analysis of active and latent forms of MMP-8 from GCF that bind to collagen.	bind
6498	2	2520	7	10	NULL	0	NULL	MMP-8	GP	latent	binds					collagen	GP				NULL	GCF	NULL	NULL	NULL	NULL	gw60_infectimmun_67_5_2319_s_228	10225890	(A) Analysis of active and latent forms of MMP-8 from GCF that bind to collagen.	bind
5936	1	2521	6	10	NULL	0	NULL	AlgZ	GP		bind					algD	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_24_7297_s_38	14645293	(A) Analysis of AlgZ binding to  algD by electrophoretic mobility shift assay.	bind
6503	1	2521	7	10	NULL	0	NULL	AlgZ	GP		binds	GP				algD	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_24_7297_s_38	14645293	(A) Analysis of AlgZ binding to  algD by electrophoretic mobility shift assay.	bind
5937	1	2523	6	10	NULL	0	NULL	P. multocida 232	Organism		pre incubated with					anti-PmOmpA	GP	mouse			NULL		NULL	NULL	NULL	NULL	gw70_microbpathogenesis_35_4_147_s_154	12946327	(A) and (B) Binding of Fn to  P. multocida 232 pre-incubated with mouse anti-PmOmpA (lanes 2 and 4), in the presence or absence  of Hp (lanes 1, and 3, respectively).	bind
5938	2	2523	6	10	NULL	0	NULL	Fn	GP		bind					statement 1	Organism				NULL		NULL	NULL	NULL	NULL	gw70_microbpathogenesis_35_4_147_s_154	12946327	(A) and (B) Binding of Fn to  P. multocida 232 pre-incubated with mouse anti-PmOmpA (lanes 2 and 4), in the presence or absence  of Hp (lanes 1, and 3, respectively).	bind
6505	1	2523	7	10	NULL	0	NULL	Fn	GP		binds					 P. multocida 232	Organism				NULL		NULL	NULL	NULL	NULL	gw70_microbpathogenesis_35_4_147_s_154	12946327	(A) and (B) Binding of Fn to  P. multocida 232 pre-incubated with mouse anti-PmOmpA (lanes 2 and 4), in the presence or absence  of Hp (lanes 1, and 3, respectively).	bind
6507	2	2523	7	10	NULL	0	NULL	 P. multocida 232	Organism		is pre-incubated with					anti-PmOmpA	GP	mouse			NULL		NULL	NULL	NULL	NULL	gw70_microbpathogenesis_35_4_147_s_154	12946327	(A) and (B) Binding of Fn to  P. multocida 232 pre-incubated with mouse anti-PmOmpA (lanes 2 and 4), in the presence or absence  of Hp (lanes 1, and 3, respectively).	bind
5939	1	2525	6	10	NULL	0	NULL	HOCl	Chemical		oxidizes					LDL	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_12_1902_s_113	11742862	(A) and analysis of HOCl-oxidized LDL released and remaining bound to heparin-Sepharose (B and C).	bind
5940	2	2525	6	10	NULL	0	NULL	LDL	Chemical	unoxidized	bind					heparin	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_12_1902_s_113	11742862	(A) and analysis of HOCl-oxidized LDL released and remaining bound to heparin-Sepharose (B and C).	bind
6511	1	2525	7	10	NULL	0	NULL	LDL	Chemical		binds to					heparin	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_12_1902_s_113	11742862	(A) and analysis of HOCl-oxidized LDL released and remaining bound to heparin-Sepharose (B and C).	bind
6512	2	2525	7	10	NULL	0	NULL	HOCl	Chemical		oxidizes					LDL	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_12_1902_s_113	11742862	(A) and analysis of HOCl-oxidized LDL released and remaining bound to heparin-Sepharose (B and C).	bind
5941	1	2528	6	10	NULL	0	NULL	[15N, 2]cTnC	GP	Ca2+ saturated	bind					cTnI	GP		1-80		NULL		NULL	NULL	NULL	NULL	gw60_febslett_469_2_168_s_143	10713265	(A) and Ca2+ saturated [15N, 2]cTnC bound to cTnI(1-80) and cTnIp at a ratio of 1:1:1.4 (B) and Ca2+ saturated [15N, 2]cTnC bound to cTnI(1-80) and cTnIp at a stoichiometry of 1:1:2.6 (C).	bind
5942	2	2528	6	10	NULL	0	NULL	[15N, 2]cTnC	GP	Ca2+ saturated	bind					cTnIp	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_469_2_168_s_143	10713265	(A) and Ca2+ saturated [15N, 2]cTnC bound to cTnI(1-80) and cTnIp at a ratio of 1:1:1.4 (B) and Ca2+ saturated [15N, 2]cTnC bound to cTnI(1-80) and cTnIp at a stoichiometry of 1:1:2.6 (C).	bind
6519	1	2528	7	10	NULL	0	NULL	[15N, 2]cTnC	GP	Ca2+ saturated	binds					cTnI	GP		1-80		NULL		NULL	NULL	NULL	NULL	gw60_febslett_469_2_168_s_143	10713265	(A) and Ca2+ saturated [15N, 2]cTnC bound to cTnI(1-80) and cTnIp at a ratio of 1:1:1.4 (B) and Ca2+ saturated [15N, 2]cTnC bound to cTnI(1-80) and cTnIp at a stoichiometry of 1:1:2.6 (C).	bind
6520	2	2528	7	10	NULL	0	NULL	[15N, 2]cTnC	GP	Ca2+ saturated	bind					cTnIp	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_469_2_168_s_143	10713265	(A) and Ca2+ saturated [15N, 2]cTnC bound to cTnI(1-80) and cTnIp at a ratio of 1:1:1.4 (B) and Ca2+ saturated [15N, 2]cTnC bound to cTnI(1-80) and cTnIp at a stoichiometry of 1:1:2.6 (C).	bind
5943	1	2529	6	10	NULL	0	NULL	CDK2	GP		bind					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_6_1321_s_47	11430833	(A) and CDK2 (B) bound to ATP are shown.	bind
6521	1	2529	7	10	NULL	0	NULL	CDK2	GP		binds to					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_6_1321_s_47	11430833	(A) and CDK2 (B) bound to ATP are shown.	bind
5944	1	2530	6	10	NULL	0	NULL	Cyclin E	GP		bind					p107	GP	full length			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5380_s_291	9710622	(A) and cyclin E (B) bind delta10N and N385, albeit less efficiently than full-length p107, but do not bind the mutant delta10N-AAA.	bind
5945	2	2530	6	10	NULL	0	NULL	Cyclin E	GP		bind		less efficiently			p107	GP	mutant	delta10N		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5380_s_291	9710622	(A) and cyclin E (B) bind delta10N and N385, albeit less efficiently than full-length p107, but do not bind the mutant delta10N-AAA.	bind
5946	3	2530	6	10	NULL	0	NULL	Cyclin E	GP		bind		less efficiently			p107	GP	mutant	N385		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5380_s_291	9710622	(A) and cyclin E (B) bind delta10N and N385, albeit less efficiently than full-length p107, but do not bind the mutant delta10N-AAA.	bind
5947	4	2530	6	10	NULL	0	NULL	Cyclin E	GP		does not bind					p107	GP	mutant	delta10N-AAA		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5380_s_291	9710622	(A) and cyclin E (B) bind delta10N and N385, albeit less efficiently than full-length p107, but do not bind the mutant delta10N-AAA.	bind
6522	1	2530	7	10	NULL	0	NULL	cyclin E	GP		bind					p107	GP		delta10N		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5380_s_291	9710622	(A) and cyclin E (B) bind delta10N and N385, albeit less efficiently than full-length p107, but do not bind the mutant delta10N-AAA.	bind
6523	2	2530	7	10	NULL	0	NULL	cyclin E	GP		bind					p107	GP		N385		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5380_s_291	9710622	(A) and cyclin E (B) bind delta10N and N385, albeit less efficiently than full-length p107, but do not bind the mutant delta10N-AAA.	bind
6524	3	2530	7	10	NULL	0	NULL	cyclin E	GP		bind					p107	GP	full-length			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5380_s_291	9710622	(A) and cyclin E (B) bind delta10N and N385, albeit less efficiently than full-length p107, but do not bind the mutant delta10N-AAA.	bind
6525	4	2530	7	10	NULL	0	NULL	cyclin E	GP		does not bind					p107	GP	mutant	delta10N-AAA		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5380_s_291	9710622	(A) and cyclin E (B) bind delta10N and N385, albeit less efficiently than full-length p107, but do not bind the mutant delta10N-AAA.	bind
6526	5	2530	7	10	NULL	0	NULL	statement 1	GP		is less efficient than					statement 3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5380_s_291	9710622	(A) and cyclin E (B) bind delta10N and N385, albeit less efficiently than full-length p107, but do not bind the mutant delta10N-AAA.	bind
6527	6	2530	7	10	NULL	0	NULL	statement 2	GP		is less efficient than					statement 3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5380_s_291	9710622	(A) and cyclin E (B) bind delta10N and N385, albeit less efficiently than full-length p107, but do not bind the mutant delta10N-AAA.	bind
5948	1	2532	6	10	NULL	0	NULL	APPA	Chemical		bind					GABAB receptors	GP	native			NULL	rat cortical membranes	NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_307_1_322_s_165	12954816	(A) and dissociation (B) of [3]APPA binding to native GABAB receptors in rat cortical membranes.	bind
6528	1	2532	7	10	NULL	0	NULL	[3]APPA	Chemical		binds to					GABAB receptors	GP	native			NULL	rat cortical membranes	NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_307_1_322_s_165	12954816	(A) and dissociation (B) of [3]APPA binding to native GABAB receptors in rat cortical membranes.	bind
5949	1	2533	6	10	NULL	0	NULL	NahR	GP		bind					PsaI	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1725_2_247_s_210	15978733	(A) and dissociation (B) phases of NahR binding  to  Psal.	bind
6529	1	2533	7	10	NULL	0	NULL	NahR	GP		binds					Psal	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1725_2_247_s_210	15978733	(A) and dissociation (B) phases of NahR binding  to  Psal.	bind
5950	1	2534	6	10	NULL	0	NULL	XylS	GP	wild type	bind		specifically	N-terminal		Om	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_4_1118_s_179	10648539	(A) and DNase I footprinting (B) showing that wt N-XylS and XylS CTD bind specifically to  Om.	bind
5951	2	2534	6	10	NULL	0	NULL	XylS	GP		bind		specifically	CTD		Om	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_4_1118_s_179	10648539	(A) and DNase I footprinting (B) showing that wt N-XylS and XylS CTD bind specifically to  Om.	bind
6530	1	2534	7	10	NULL	0	NULL	XylS 	GP	wt	bind		specifically	N-terminal		Om	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_4_1118_s_179	10648539	(A) and DNase I footprinting (B) showing that wt N-XylS and XylS CTD bind specifically to  Om.	bind
6531	2	2534	7	10	NULL	0	NULL	XylS	GP		bind		specifically	CTD		Om	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_4_1118_s_179	10648539	(A) and DNase I footprinting (B) showing that wt N-XylS and XylS CTD bind specifically to  Om.	bind
5952	1	2535	6	10	NULL	0	NULL	FbsA	GP		bind					fibrinogen	GP	native			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_6_3495_s_210	15155657	(A) and dot blot experiments to detect binding of the FbsA and FbsB  fusion proteins to native fibrinogen (B).	bind
5953	2	2535	6	10	NULL	0	NULL	FbsB	GP		bind					fibrinogen	GP	native			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_6_3495_s_210	15155657	(A) and dot blot experiments to detect binding of the FbsA and FbsB  fusion proteins to native fibrinogen (B).	bind
46336	3	2535	6	10	NULL	0	NULL	FbsA	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_6_3495_s_210	15155657	(A) and dot blot experiments to detect binding of the FbsA and FbsB  fusion proteins to native fibrinogen (B).	bind
46337	4	2535	6	10	NULL	0	NULL	FbsB	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_6_3495_s_210	15155657	(A) and dot blot experiments to detect binding of the FbsA and FbsB  fusion proteins to native fibrinogen (B).	bind
6532	1	2535	7	10	NULL	0	NULL	FbsA	GP		bind					fibrinogen	GP	native			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_6_3495_s_210	15155657	(A) and dot blot experiments to detect binding of the FbsA and FbsB  fusion proteins to native fibrinogen (B).	bind
6533	2	2535	7	10	NULL	0	NULL	FbsB	GP		bind					fibrinogen	GP	native			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_6_3495_s_210	15155657	(A) and dot blot experiments to detect binding of the FbsA and FbsB  fusion proteins to native fibrinogen (B).	bind
46338	3	2535	7	10	NULL	0	NULL	FbsA	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_6_3495_s_210	15155657	(A) and dot blot experiments to detect binding of the FbsA and FbsB  fusion proteins to native fibrinogen (B).	bind
46339	4	2535	7	10	NULL	0	NULL	FbsB	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_6_3495_s_210	15155657	(A) and dot blot experiments to detect binding of the FbsA and FbsB  fusion proteins to native fibrinogen (B).	bind
5954	1	2537	6	10	NULL	0	NULL	endothelin-1	GP		bind					endothelin receptor 	GP	atypical			NULL	primary rat astrocytes	NULL	NULL	NULL	NULL	gw60_neuroscience_91_3_1067_s_305	10391484	(A) and ET(B) specific ligands synergistically antagonize endothelin-1 binding to an atypical endothelin receptor in primary rat astrocytes.	bind
5955	2	2537	6	10	NULL	0	NULL	ET specific ligands	Chemical		antagonize		synergistically			statement 1	Process				NULL	primary rat astrocytes	NULL	NULL	NULL	NULL	gw60_neuroscience_91_3_1067_s_305	10391484	(A) and ET(B) specific ligands synergistically antagonize endothelin-1 binding to an atypical endothelin receptor in primary rat astrocytes.	bind
6534	1	2537	7	10	NULL	0	NULL	endothelin-1	GP		bind					endothelin receptor	GP	atypical			NULL	primary rat astrocytes	NULL	NULL	NULL	NULL	gw60_neuroscience_91_3_1067_s_305	10391484	(A) and ET(B) specific ligands synergistically antagonize endothelin-1 binding to an atypical endothelin receptor in primary rat astrocytes.	bind
6535	2	2537	7	10	NULL	0	NULL	ET specific ligands	Chemical		antagonize		synergistically			statement 1	Process				NULL	primary rat astrocytes	NULL	NULL	NULL	NULL	gw60_neuroscience_91_3_1067_s_305	10391484	(A) and ET(B) specific ligands synergistically antagonize endothelin-1 binding to an atypical endothelin receptor in primary rat astrocytes.	bind
7861	1	2538	6	10	NULL	0	NULL	Fn	GP		bind					lactobacillus	Organism				NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_206_1_31_s_129	11786253	(A) and Fn (B) binding by  Lactobacillus.	bind
6536	1	2538	7	10	NULL	0	NULL	Fn 	GP		binds to					Lactobacillus	Organism				NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_206_1_31_s_129	11786253	(A) and Fn (B) binding by  Lactobacillus.	bind
5956	1	2541	6	10	NULL	0	NULL	SREBP-1	GP		bind					malic enzyme gene	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_43_8_1220_s_84	12177166	(A) and gel mobility shift assay for binding of SREBP-1 to the malic enzyme gene promoter (B).	bind
6537	1	2541	7	10	NULL	0	NULL	SREBP-1	GP		binds to					malic enzyme gene 	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_43_8_1220_s_84	12177166	(A) and gel mobility shift assay for binding of SREBP-1 to the malic enzyme gene promoter (B).	bind
5958	1	2543	6	10	NULL	0	NULL	Gpp(NH)p	GP		bind					ARF1	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_487_2_252_s_132	11150519	(A) and Gpp(NH)p (B) bound conformations of ARF1.	bind
6539	1	2543	7	10	NULL	0	NULL	Gpp(NH)p	GP		bind					ARF1	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_487_2_252_s_132	11150519	(A) and Gpp(NH)p (B) bound conformations of ARF1.	bind
5959	1	2544	6	10	NULL	0	NULL	progesterone	GP		inhibits					pentazocine	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_289_1_251_s_274	10087012	(A) and inhibition of [3]-(+)-pentazocine binding by progesterone (B).	bind
6540	1	2544	7	10	NULL	0	NULL	progesterone	GP		inhibits					pentazocine	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_289_1_251_s_274	10087012	(A) and inhibition of [3]-(+)-pentazocine binding by progesterone (B).	bind
5960	1	2545	6	10	NULL	0	NULL	actininn2	GP		bind		non-specifically			Protein A	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_473_2_188_s_229	10812072	(A) and lane 1 in (B) and (C) exclude non-specific binding of  actininn2 and Kv1.5 to the protein A-Sepharose.	bind
5961	2	2545	6	10	NULL	0	NULL	Kv1.5	GP		bind		non-specifically			Protein A	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_473_2_188_s_229	10812072	(A) and lane 1 in (B) and (C) exclude non-specific binding of  actininn2 and Kv1.5 to the protein A-Sepharose.	bind
6541	1	2545	7	10	NULL	0	NULL	actininn2	GP		bind		non-specifically			protein A	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_473_2_188_s_229	10812072	(A) and lane 1 in (B) and (C) exclude non-specific binding of  actininn2 and Kv1.5 to the protein A-Sepharose.	bind
6542	2	2545	7	10	NULL	0	NULL	Kv1.5	GP		bind		non-specifically			protein A	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_473_2_188_s_229	10812072	(A) and lane 1 in (B) and (C) exclude non-specific binding of  actininn2 and Kv1.5 to the protein A-Sepharose.	bind
5962	1	2546	6	10	NULL	0	NULL	mt-CMT1	GP		bind					GST-SAHH	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1590_1_93_s_155	12063172	(A) and mt-CMT1 (B) were bound by the GST-SAHH fusion protein but not by GST alone, indicating that binding of xCMT1 to xSAHH was independent of the tag sequence used.	bind
5963	2	2546	6	10	NULL	0	NULL	mt-CMT1	GP		does not bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1590_1_93_s_155	12063172	(A) and mt-CMT1 (B) were bound by the GST-SAHH fusion protein but not by GST alone, indicating that binding of xCMT1 to xSAHH was independent of the tag sequence used.	bind
5964	3	2546	6	10	NULL	0	NULL	statement 1	Process		is independent of					tag sequence	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1590_1_93_s_155	12063172	(A) and mt-CMT1 (B) were bound by the GST-SAHH fusion protein but not by GST alone, indicating that binding of xCMT1 to xSAHH was independent of the tag sequence used.	bind
46359	4	2546	6	10	NULL	0	NULL	GST-SAHH	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1590_1_93_s_155	12063172	(A) and mt-CMT1 (B) were bound by the GST-SAHH fusion protein but not by GST alone, indicating that binding of xCMT1 to xSAHH was independent of the tag sequence used.	bind
6543	1	2546	7	10	NULL	0	NULL	mt-CMT1	GP		binds					GST-SAHH	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1590_1_93_s_155	12063172	(A) and mt-CMT1 (B) were bound by the GST-SAHH fusion protein but not by GST alone, indicating that binding of xCMT1 to xSAHH was independent of the tag sequence used.	bind
6544	2	2546	7	10	NULL	0	NULL	 mt-CMT1	GP		does not bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1590_1_93_s_155	12063172	(A) and mt-CMT1 (B) were bound by the GST-SAHH fusion protein but not by GST alone, indicating that binding of xCMT1 to xSAHH was independent of the tag sequence used.	bind
6545	3	2546	7	10	NULL	0	NULL	statement 1	Process		is independent of					tag sequence	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1590_1_93_s_155	12063172	(A) and mt-CMT1 (B) were bound by the GST-SAHH fusion protein but not by GST alone, indicating that binding of xCMT1 to xSAHH was independent of the tag sequence used.	bind
46360	4	2546	7	10	NULL	0	NULL	GST-SAHH	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1590_1_93_s_155	12063172	(A) and mt-CMT1 (B) were bound by the GST-SAHH fusion protein but not by GST alone, indicating that binding of xCMT1 to xSAHH was independent of the tag sequence used.	bind
5965	1	2547	6	10	NULL	0	NULL	E1A protein	GP	mutant	bind		selectively			p300	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_510_1_50_s_167	11755530	(A) and neurite outgrowth (B) are inhibited by an E1A mutant protein that selectively binds p300.	bind
5966	2	2547	6	10	NULL	0	NULL	E1A protein	GP	mutant	inhibits					neurite outgrowth	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_510_1_50_s_167	11755530	(A) and neurite outgrowth (B) are inhibited by an E1A mutant protein that selectively binds p300.	bind
6546	1	2547	7	10	NULL	0	NULL	E1A protein	GP	mutant	binds to 		selectively			p300	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_510_1_50_s_167	11755530	(A) and neurite outgrowth (B) are inhibited by an E1A mutant protein that selectively binds p300.	bind
6547	2	2547	7	10	NULL	0	NULL	neurite outgrowth	Process		is inhibited by					E1A protein	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_febslett_510_1_50_s_167	11755530	(A) and neurite outgrowth (B) are inhibited by an E1A mutant protein that selectively binds p300.	bind
5967	1	2549	6	10	NULL	0	NULL	eIF4G2	GP		bind					eIF1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_15_5431_s_120	12861028	(A) and point mutations (B) on eIF4G2 binding to eIF1  and eIF5.	bind
5968	2	2549	6	10	NULL	0	NULL	eIF4G2	GP		bind					eIF5	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_15_5431_s_120	12861028	(A) and point mutations (B) on eIF4G2 binding to eIF1  and eIF5.	bind
6548	1	2549	7	10	NULL	0	NULL	eIF4G2	GP		binds to					eIF1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_15_5431_s_120	12861028	(A) and point mutations (B) on eIF4G2 binding to eIF1  and eIF5.	bind
6549	2	2549	7	10	NULL	0	NULL	eIF4G2	GP		binds to					eIF5	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_15_5431_s_120	12861028	(A) and point mutations (B) on eIF4G2 binding to eIF1  and eIF5.	bind
5969	1	2550	6	10	NULL	0	NULL	eIF4G2	GP		bind					eIF1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_15_5431_s_120	12861028	(A) and point mutations (B) on eIF4G2 binding to eIF1 and eIF5.	bind
5970	2	2550	6	10	NULL	0	NULL	eIF4G2	GP		bind					eIF5	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_15_5431_s_120	12861028	(A) and point mutations (B) on eIF4G2 binding to eIF1 and eIF5.	bind
7862	1	2551	6	10	NULL	0	NULL	Poly(g) sequences	NucleicAcid		inserted into					coding sequences	NucleicAcid	yeast;;upstream of			NULL		NULL	NULL	NULL	NULL	gw60_genetics_152_1_101_s_331	10224246	(A) and poly(G) sequences inserted upstream of the coding sequences stimulate transcription in yeast in the absence of the binding of known transcription factors.	bind
7863	2	2551	6	10	NULL	0	NULL	statement 1	Process		stimulate					transcription	Process	yeast			NULL		NULL	NULL	NULL	NULL	gw60_genetics_152_1_101_s_331	10224246	(A) and poly(G) sequences inserted upstream of the coding sequences stimulate transcription in yeast in the absence of the binding of known transcription factors.	bind
7864	3	2551	6	10	NULL	0	NULL	statement 2	Process		occurs in absence of					transcription factors	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_genetics_152_1_101_s_331	10224246	(A) and poly(G) sequences inserted upstream of the coding sequences stimulate transcription in yeast in the absence of the binding of known transcription factors.	bind
6550	1	2551	7	10	NULL	0	NULL	poly(G) sequences	NucleicAcid		is inserted into					coding sequences	NucleicAcid	yeast;;upstream of			NULL		NULL	NULL	NULL	NULL	gw60_genetics_152_1_101_s_331	10224246	(A) and poly(G) sequences inserted upstream of the coding sequences stimulate transcription in yeast in the absence of the binding of known transcription factors.	bind
6551	2	2551	7	10	NULL	0	NULL	statement 1	Process		stimulate					transcription 	Process	yeast			NULL		NULL	NULL	NULL	NULL	gw60_genetics_152_1_101_s_331	10224246	(A) and poly(G) sequences inserted upstream of the coding sequences stimulate transcription in yeast in the absence of the binding of known transcription factors.	bind
6552	3	2551	7	10	NULL	0	NULL	statement 2	Process		occurs in the absence of 					transcription factors	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_genetics_152_1_101_s_331	10224246	(A) and poly(G) sequences inserted upstream of the coding sequences stimulate transcription in yeast in the absence of the binding of known transcription factors.	bind
5971	1	2553	6	10	NULL	0	NULL	125I-[Tyr3]MP	GP		bind					HSR	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_57_6_1235_s_191	10825395	(A) and Scatchard (B) plots of 125I-[Tyr3]MP binding to HSR.	bind
6553	1	2553	7	10	NULL	0	NULL	125I-[Tyr3]MP	GP		binds					HSR	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_57_6_1235_s_191	10825395	(A) and Scatchard (B) plots of 125I-[Tyr3]MP binding to HSR.	bind
61567	1	2554	6	10	NULL	0	NULL	CFT	Chemical		bind					DAT	GP	WT			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_56_2_434_s_146	10419565	(A) and Scatchard analysis of [3]CFT binding activity (B) with the WT DAT (top) and two representative DAT mutants 3F155A (middle) and 7F361A (bottom).	bind
61568	2	2554	6	10	NULL	0	NULL	CFT	Chemical		bind					DAT	GP	mutant	3F155A		NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_56_2_434_s_146	10419565	(A) and Scatchard analysis of [3]CFT binding activity (B) with the WT DAT (top) and two representative DAT mutants 3F155A (middle) and 7F361A (bottom).	bind
61569	3	2554	6	10	NULL	0	NULL	CFT	Chemical		bind					DAT	GP	mutant	7F361A		NULL		0	NULL	NULL	NULL	gw60_molpharmacol_56_2_434_s_146	10419565	(A) and Scatchard analysis of [3]CFT binding activity (B) with the WT DAT (top) and two representative DAT mutants 3F155A (middle) and 7F361A (bottom).	bind
6554	1	2554	7	10	NULL	0	NULL	[3]CFT	Chemical		binds					DAT	GP	WT			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_56_2_434_s_146	10419565	(A) and Scatchard analysis of [3]CFT binding activity (B) with the WT DAT (top) and two representative DAT mutants 3F155A (middle) and 7F361A (bottom).	bind
6555	2	2554	7	10	NULL	0	NULL	[3]CFT	Chemical		binds					DAT	GP	mutant	3F155A		NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_56_2_434_s_146	10419565	(A) and Scatchard analysis of [3]CFT binding activity (B) with the WT DAT (top) and two representative DAT mutants 3F155A (middle) and 7F361A (bottom).	bind
6556	3	2554	7	10	NULL	0	NULL	[3]CFT	Chemical		binds					DAT	GP	mutant	 7F361A		NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_56_2_434_s_146	10419565	(A) and Scatchard analysis of [3]CFT binding activity (B) with the WT DAT (top) and two representative DAT mutants 3F155A (middle) and 7F361A (bottom).	bind
5972	1	2557	6	10	NULL	0	NULL	SLM-2	GP		bind					poly(G) homopolymeric RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_52_54398_s_177	15471878	(A) and SLM-2 bound poly(G) homopolymeric RNA when cotransfections were performed with the empty expression vector.	bind
6815	1	2557	7	10	NULL	0	NULL	SLM-2	GP		bind					poly(G) homopolymeric RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_52_54398_s_177	15471878	(A) and SLM-2 bound poly(G) homopolymeric RNA when cotransfections were performed with the empty expression vector.	bind
5974	1	2558	6	10	NULL	0	NULL	puroA	GP		bind					POPG SUV	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_16_4938_s_176	12897014	(A) and Stern-Volmer plots (B) for 2 muM puroA bound to POPG SUVs (lines a) and to POPC SUVs (lines b) and in buffer (lines c).	bind
5975	2	2558	6	10	NULL	0	NULL	puroA	GP		bind					POPC SUV	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_16_4938_s_176	12897014	(A) and Stern-Volmer plots (B) for 2 muM puroA bound to POPG SUVs (lines a) and to POPC SUVs (lines b) and in buffer (lines c).	bind
6816	1	2558	7	10	NULL	0	NULL	puroA	GP		binds					POPG SUVs	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_16_4938_s_176	12897014	(A) and Stern-Volmer plots (B) for 2 muM puroA bound to POPG SUVs (lines a) and to POPC SUVs (lines b) and in buffer (lines c).	bind
6818	2	2558	7	10	NULL	0	NULL	puroA	GP		binds					POPC SUVs	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_16_4938_s_176	12897014	(A) and Stern-Volmer plots (B) for 2 muM puroA bound to POPG SUVs (lines a) and to POPC SUVs (lines b) and in buffer (lines c).	bind
7865	1	2560	6	10	NULL	0	NULL	Cn-I	GP		bind					CRL 639	GP	L. acidophilus			NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_206_1_31_s_141	11786253	(A) and temperature (B) on binding of Cn-I ( ) and Fn ( ) by  L. acidophilus CRL 639.	bind
7866	2	2560	6	10	NULL	0	NULL	Fn	GP		bind					CRL 639	GP	L. acidophilus			NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_206_1_31_s_141	11786253	(A) and temperature (B) on binding of Cn-I ( ) and Fn ( ) by  L. acidophilus CRL 639.	bind
6823	1	2560	7	10	NULL	0	NULL	Cn-I	GP		binds					CRL 639	GP	L. acidophilus 			NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_206_1_31_s_141	11786253	(A) and temperature (B) on binding of Cn-I ( ) and Fn ( ) by  L. acidophilus CRL 639.	bind
6824	2	2560	7	10	NULL	0	NULL	Fn	GP		binds					CRL 639	GP	L. acidophilus 			NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_206_1_31_s_141	11786253	(A) and temperature (B) on binding of Cn-I ( ) and Fn ( ) by  L. acidophilus CRL 639.	bind
5976	1	2562	6	10	NULL	0	NULL				bind			TM helices		Chl molecules	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_45_44542_s_5	12923171	(A) and the third (C) transmembrane (TM) helices that binds 6 Chl molecules and two carotenoids is conserved structurally, whereas the interface between the first and the second TM helices and the outer surface of the second TM helix differ significantly among the LHCI and LHCII polypeptides.	bind
5977	2	2562	6	10	NULL	0	NULL				bind			transmembrane helices		carotenoids	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_45_44542_s_5	12923171	(A) and the third (C) transmembrane (TM) helices that binds 6 Chl molecules and two carotenoids is conserved structurally, whereas the interface between the first and the second TM helices and the outer surface of the second TM helix differ significantly among the LHCI and LHCII polypeptides.	bind
5978	3	2562	6	10	NULL	0	NULL	TM helics	AminoAcid		is					transmembrane helics	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_45_44542_s_5	12923171	(A) and the third (C) transmembrane (TM) helices that binds 6 Chl molecules and two carotenoids is conserved structurally, whereas the interface between the first and the second TM helices and the outer surface of the second TM helix differ significantly among the LHCI and LHCII polypeptides.	bind
7867	4	2562	6	10	NULL	0	NULL	LHCI polypeptide	GP		differ		significantly	first TM helices		LHCII polypeptide	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_45_44542_s_5	12923171	(A) and the third (C) transmembrane (TM) helices that binds 6 Chl molecules and two carotenoids is conserved structurally, whereas the interface between the first and the second TM helices and the outer surface of the second TM helix differ significantly among the LHCI and LHCII polypeptides.	bind
7868	5	2562	6	10	NULL	0	NULL	LHCI polypeptide	GP		differ		significantly	second TM helices		LHCII polypeptide	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_45_44542_s_5	12923171	(A) and the third (C) transmembrane (TM) helices that binds 6 Chl molecules and two carotenoids is conserved structurally, whereas the interface between the first and the second TM helices and the outer surface of the second TM helix differ significantly among the LHCI and LHCII polypeptides.	bind
7869	6	2562	6	10	NULL	0	NULL	LHCI polypeptide	GP		differ		significantly	outer surface of the second TM helix		LHCII polypeptide	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_45_44542_s_5	12923171	(A) and the third (C) transmembrane (TM) helices that binds 6 Chl molecules and two carotenoids is conserved structurally, whereas the interface between the first and the second TM helices and the outer surface of the second TM helix differ significantly among the LHCI and LHCII polypeptides.	bind
6826	1	2562	7	10	NULL	0	NULL	 			binds			transmembrane helices		Chl molecules	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_45_44542_s_5	12923171	(A) and the third (C) transmembrane (TM) helices that binds 6 Chl molecules and two carotenoids is conserved structurally, whereas the interface between the first and the second TM helices and the outer surface of the second TM helix differ significantly among the LHCI and LHCII polypeptides.	bind
6827	2	2562	7	10	NULL	0	NULL				binds			transmembrane helices		carotenoids	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_45_44542_s_5	12923171	(A) and the third (C) transmembrane (TM) helices that binds 6 Chl molecules and two carotenoids is conserved structurally, whereas the interface between the first and the second TM helices and the outer surface of the second TM helix differ significantly among the LHCI and LHCII polypeptides.	bind
6904	3	2562	7	10	NULL	0	NULL	TM helics	AminoAcid		is					transmembrane helics	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_45_44542_s_5	12923171	(A) and the third (C) transmembrane (TM) helices that binds 6 Chl molecules and two carotenoids is conserved structurally, whereas the interface between the first and the second TM helices and the outer surface of the second TM helix differ significantly among the LHCI and LHCII polypeptides.	bind
7194	5	2562	7	10	NULL	0	NULL	LHCI polypeptides	GP	Interface of 	differ		significantly	first TM helix		LHCII polypeptides	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_45_44542_s_5	12923171	(A) and the third (C) transmembrane (TM) helices that binds 6 Chl molecules and two carotenoids is conserved structurally, whereas the interface between the first and the second TM helices and the outer surface of the second TM helix differ significantly among the LHCI and LHCII polypeptides.	bind
7196	6	2562	7	10	NULL	0	NULL	LHCI polypeptides	GP	Interface of	differ		significantly	second TM helix		LHCII polypeptides	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_45_44542_s_5	12923171	(A) and the third (C) transmembrane (TM) helices that binds 6 Chl molecules and two carotenoids is conserved structurally, whereas the interface between the first and the second TM helices and the outer surface of the second TM helix differ significantly among the LHCI and LHCII polypeptides.	bind
7271	4	2562	7	10	NULL	0	NULL	LHCI polypeptides	GP		differ		significantly	outer surface of second TM helix		LHCII polypeptides	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_45_44542_s_5	12923171	(A) and the third (C) transmembrane (TM) helices that binds 6 Chl molecules and two carotenoids is conserved structurally, whereas the interface between the first and the second TM helices and the outer surface of the second TM helix differ significantly among the LHCI and LHCII polypeptides.	bind
5979	1	2563	6	10	NULL	0	NULL	transferrin	GP		bind					rTbpB proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_9_4183_s_218	9712766	(A) and transferrin binding of rTbpB proteins (B).	bind
6833	1	2563	7	10	NULL	0	NULL	transferrin	GP		binds					rTbpB proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_9_4183_s_218	9712766	(A) and transferrin binding of rTbpB proteins (B).	bind
5980	1	2564	6	10	NULL	0	NULL	TTF-1	GP		bind					CaSR-C	GP			TTF-1 element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7410_s_263	9819427	(A) and TTF-1 binding to the CaSR-C TTF-1 element (B) are decreased by the ATP- or A23187-increased the internal Ca2+ signal, and kinase C activation can synergistically increase the Ca2+ signal effect.	bind
5981	2	2564	6	10	NULL	0	NULL	ATP	Chemical		decreases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7410_s_263	9819427	(A) and TTF-1 binding to the CaSR-C TTF-1 element (B) are decreased by the ATP- or A23187-increased the internal Ca2+ signal, and kinase C activation can synergistically increase the Ca2+ signal effect.	bind
5982	3	2564	6	10	NULL	0	NULL	A23187	Chemical		increased					Ca+2 signal	Process	internal			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7410_s_263	9819427	(A) and TTF-1 binding to the CaSR-C TTF-1 element (B) are decreased by the ATP- or A23187-increased the internal Ca2+ signal, and kinase C activation can synergistically increase the Ca2+ signal effect.	bind
5983	4	2564	6	10	NULL	0	NULL	A23187	Chemical		increased					kinase C	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7410_s_263	9819427	(A) and TTF-1 binding to the CaSR-C TTF-1 element (B) are decreased by the ATP- or A23187-increased the internal Ca2+ signal, and kinase C activation can synergistically increase the Ca2+ signal effect.	bind
6212	5	2564	6	10	NULL	0	NULL	statement 3	Process		act synergistically with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7410_s_263	9819427	(A) and TTF-1 binding to the CaSR-C TTF-1 element (B) are decreased by the ATP- or A23187-increased the internal Ca2+ signal, and kinase C activation can synergistically increase the Ca2+ signal effect.	bind
6213	6	2564	6	10	NULL	0	NULL	statement 5	Process		increase					Ca+2 signal effect	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7410_s_263	9819427	(A) and TTF-1 binding to the CaSR-C TTF-1 element (B) are decreased by the ATP- or A23187-increased the internal Ca2+ signal, and kinase C activation can synergistically increase the Ca2+ signal effect.	bind
6834	1	2564	7	10	NULL	0	NULL	TTF-1	GP		bind					CaSR-C	GP			TTF-1 element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7410_s_263	9819427	(A) and TTF-1 binding to the CaSR-C TTF-1 element (B) are decreased by the ATP- or A23187-increased the internal Ca2+ signal, and kinase C activation can synergistically increase the Ca2+ signal effect.	bind
6835	2	2564	7	10	NULL	0	NULL	statement 1	Process		is decreased by					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7410_s_263	9819427	(A) and TTF-1 binding to the CaSR-C TTF-1 element (B) are decreased by the ATP- or A23187-increased the internal Ca2+ signal, and kinase C activation can synergistically increase the Ca2+ signal effect.	bind
6836	3	2564	7	10	NULL	0	NULL	A23187	Chemical		increased					Ca2+ signal	Process	internal 			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7410_s_263	9819427	(A) and TTF-1 binding to the CaSR-C TTF-1 element (B) are decreased by the ATP- or A23187-increased the internal Ca2+ signal, and kinase C activation can synergistically increase the Ca2+ signal effect.	bind
7902	5	2564	7	10	NULL	0	NULL	A23187	Chemical		increased					Kinase C	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7410_s_263	9819427	(A) and TTF-1 binding to the CaSR-C TTF-1 element (B) are decreased by the ATP- or A23187-increased the internal Ca2+ signal, and kinase C activation can synergistically increase the Ca2+ signal effect.	bind
7909	6	2564	7	10	NULL	0	NULL	statement 5	Process		act synergistically with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7410_s_263	9819427	(A) and TTF-1 binding to the CaSR-C TTF-1 element (B) are decreased by the ATP- or A23187-increased the internal Ca2+ signal, and kinase C activation can synergistically increase the Ca2+ signal effect.	bind
5984	1	2565	6	10	NULL	0	NULL	VLDL	Chemical		bind					Sf9-CLA-1 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2341_s_172	9409200	(A) and VLDL (B) binding to Sf9-CLA-1 cells.	bind
6838	1	2565	7	10	NULL	0	NULL	VLDL 	Chemical		binds					Sf9-CLA-1 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2341_s_172	9409200	(A) and VLDL (B) binding to Sf9-CLA-1 cells.	bind
5985	1	2566	6	10	NULL	0	NULL	PlyA	GP	recombinant	bind		specifically			sphingomyelin	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1679_1_65_s_161	15245918	(A) and Western immunoblotting (B) for recombinant PlyA, and sphingomyelin-specific  binding of recombinant PlyA (C).	bind
6839	1	2566	7	10	NULL	0	NULL	sphingomyelin	Chemical		binds		specifically			PlyA	GP	recombinant			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1679_1_65_s_161	15245918	(A) and Western immunoblotting (B) for recombinant PlyA, and sphingomyelin-specific  binding of recombinant PlyA (C).	bind
5986	1	2567	6	10	NULL	0	NULL	hSNF5/INI1	GP	FLAG-tagged	bind					protein	GP	myc-tagged			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_7050_s_258	10490642	(A) Anti-FLAG Western blot of anti-myc immunoprecipitates showing the amount of coimmunoprecipitated FLAG-tagged hSNF5/INI1 (lanes 1 to 7) and FLAG-tagged hSNF5/INI1 and GADD34 (lane 8) proteins bound to the myc-tagged proteins expressed in the transfections described below.	bind
5987	2	2567	6	10	NULL	0	NULL	GADD34	GP	FLAG-tagged	bind					protein	GP	myc-tagged			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_7050_s_258	10490642	(A) Anti-FLAG Western blot of anti-myc immunoprecipitates showing the amount of coimmunoprecipitated FLAG-tagged hSNF5/INI1 (lanes 1 to 7) and FLAG-tagged hSNF5/INI1 and GADD34 (lane 8) proteins bound to the myc-tagged proteins expressed in the transfections described below.	bind
6840	1	2567	7	10	NULL	0	NULL	hSNF5/INI1	GP	FLAG-tagged	binds					protein	GP	myc-tagged			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_7050_s_258	10490642	(A) Anti-FLAG Western blot of anti-myc immunoprecipitates showing the amount of coimmunoprecipitated FLAG-tagged hSNF5/INI1 (lanes 1 to 7) and FLAG-tagged hSNF5/INI1 and GADD34 (lane 8) proteins bound to the myc-tagged proteins expressed in the transfections described below.	bind
7912	2	2567	7	10	NULL	0	NULL	GADD34	GP	FLAG-tagged	bind					protein	GP	myc-tagged			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_7050_s_258	10490642	(A) Anti-FLAG Western blot of anti-myc immunoprecipitates showing the amount of coimmunoprecipitated FLAG-tagged hSNF5/INI1 (lanes 1 to 7) and FLAG-tagged hSNF5/INI1 and GADD34 (lane 8) proteins bound to the myc-tagged proteins expressed in the transfections described below.	bind
6841	1	2568	7	NULL	NULL	0	NULL	IRS	NULL		is	NULL				anti-TX0016 immune serum	NULL				NULL		0	NULL	NULL	NULL	gw60_femsimmunolmedmic_28_4_291_s_181	10891652	(A) anti-TX0016 immune serum (IRS), pre-immune serum (PRS), or immune serum adsorbed with either TX0016 or a phagocytosis-susceptible strain of  E. faecium (RLA-3), or (B) IRS alone or with purified carbohydrate or a surface protein Zwittergent extract from TX0016, and exposed to PMNs as in  Fig. 1, and data are presented as the number of bacteria bound per PMN (mean+S.E.M.,  n=3-7).	bind
6842	2	2568	7	NULL	NULL	0	NULL	PRS	NULL		is	NULL				pre-immune serum 	NULL				NULL		0	NULL	NULL	NULL	gw60_femsimmunolmedmic_28_4_291_s_181	10891652	(A) anti-TX0016 immune serum (IRS), pre-immune serum (PRS), or immune serum adsorbed with either TX0016 or a phagocytosis-susceptible strain of  E. faecium (RLA-3), or (B) IRS alone or with purified carbohydrate or a surface protein Zwittergent extract from TX0016, and exposed to PMNs as in  Fig. 1, and data are presented as the number of bacteria bound per PMN (mean+S.E.M.,  n=3-7).	bind
5988	1	2569	6	10	NULL	0	NULL	AP1 protein	GP		bind									AP1 response element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4522_s_207	12052862	(A) AP1 protein binding to the AP1 response element.	bind
6843	1	2569	7	10	NULL	0	NULL	AP1 protein	GP		binds									AP1 response element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4522_s_207	12052862	(A) AP1 protein binding to the AP1 response element.	bind
5989	1	2570	6	10	NULL	0	NULL	Apg-2	GP		bind					ZO-1	GP		SH3 domain		NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molbiolcell_17_3_1322_s_106	16407410	(A) Apg-2 binds to the SH3 domain  of ZO-1 in vitro.	bind
6844	1	2570	7	10	NULL	0	NULL	Apg-2 	GP		binds					ZO-1	GP		SH3 domain		NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molbiolcell_17_3_1322_s_106	16407410	(A) Apg-2 binds to the SH3 domain  of ZO-1 in vitro.	bind
5990	1	2571	6	10	NULL	0	NULL	PABP	GP		bind					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_3_479_s_32	10882133	(A) appears to stimulate cap-dependent translation through a mechanism involving protein-protein interactions between PABP, eIF4G, and thecap binding protein eIF4E (  Tarun and Sachs 1997  ; Imataka et al. 1998  ).	bind
5991	2	2571	6	10	NULL	0	NULL	eIF4G	GP		bind					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_3_479_s_32	10882133	(A) appears to stimulate cap-dependent translation through a mechanism involving protein-protein interactions between PABP, eIF4G, and thecap binding protein eIF4E (  Tarun and Sachs 1997  ; Imataka et al. 1998  ).	bind
5992	3	2571	6	10	NULL	0	NULL	statement 1	Process		stimulate					cap-dependent translation	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_3_479_s_32	10882133	(A) appears to stimulate cap-dependent translation through a mechanism involving protein-protein interactions between PABP, eIF4G, and thecap binding protein eIF4E (  Tarun and Sachs 1997  ; Imataka et al. 1998  ).	bind
7870	4	2571	6	10	NULL	0	NULL	statement 2	Process		stimulate					cap-dependent translation	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_3_479_s_32	10882133	(A) appears to stimulate cap-dependent translation through a mechanism involving protein-protein interactions between PABP, eIF4G, and thecap binding protein eIF4E (  Tarun and Sachs 1997  ; Imataka et al. 1998  ).	bind
46361	5	2571	6	10	NULL	0	NULL	eIF4E	GP		is a type of					cap binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_3_479_s_32	10882133	(A) appears to stimulate cap-dependent translation through a mechanism involving protein-protein interactions between PABP, eIF4G, and thecap binding protein eIF4E (  Tarun and Sachs 1997  ; Imataka et al. 1998  ).	bind
6845	1	2571	7	10	NULL	0	NULL	PABP	GP		binds					eIF4G	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_3_479_s_32	10882133	(A) appears to stimulate cap-dependent translation through a mechanism involving protein-protein interactions between PABP, eIF4G, and thecap binding protein eIF4E (  Tarun and Sachs 1997  ; Imataka et al. 1998  ).	bind
6846	2	2571	7	10	NULL	0	NULL	PABP	GP		binds					eIF4E 	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_3_479_s_32	10882133	(A) appears to stimulate cap-dependent translation through a mechanism involving protein-protein interactions between PABP, eIF4G, and thecap binding protein eIF4E (  Tarun and Sachs 1997  ; Imataka et al. 1998  ).	bind
6847	3	2571	7	10	NULL	0	NULL	 eIF4G	GP		binds					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_3_479_s_32	10882133	(A) appears to stimulate cap-dependent translation through a mechanism involving protein-protein interactions between PABP, eIF4G, and thecap binding protein eIF4E (  Tarun and Sachs 1997  ; Imataka et al. 1998  ).	bind
6848	4	2571	7	10	NULL	0	NULL	statement 1	Process		stimulate					cap-dependent translation 	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_3_479_s_32	10882133	(A) appears to stimulate cap-dependent translation through a mechanism involving protein-protein interactions between PABP, eIF4G, and thecap binding protein eIF4E (  Tarun and Sachs 1997  ; Imataka et al. 1998  ).	bind
6849	5	2571	7	10	NULL	0	NULL	statement 2	Process		stimulate					cap-dependent translation 	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_3_479_s_32	10882133	(A) appears to stimulate cap-dependent translation through a mechanism involving protein-protein interactions between PABP, eIF4G, and thecap binding protein eIF4E (  Tarun and Sachs 1997  ; Imataka et al. 1998  ).	bind
6850	6	2571	7	10	NULL	0	NULL	statement 3	Process		stimulate					cap-dependent translation 	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_3_479_s_32	10882133	(A) appears to stimulate cap-dependent translation through a mechanism involving protein-protein interactions between PABP, eIF4G, and thecap binding protein eIF4E (  Tarun and Sachs 1997  ; Imataka et al. 1998  ).	bind
46362	7	2571	7	10	NULL	0	NULL	eIF4E	GP		is a type of					cap binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_3_479_s_32	10882133	(A) appears to stimulate cap-dependent translation through a mechanism involving protein-protein interactions between PABP, eIF4G, and thecap binding protein eIF4E (  Tarun and Sachs 1997  ; Imataka et al. 1998  ).	bind
5993	1	2573	6	10	NULL	0	NULL	Arp8	GP		bind		preferentially			H3	GP				NULL	in solution	NULL	NULL	NULL	NULL	gw60_molcell_12_1_147_s_188	12887900	(A) Arp8 preferentially binds to H3 and H4 in solution.	bind
5994	2	2573	6	10	NULL	0	NULL	Arp8	GP		bind		preferentially			H4	GP				NULL	in solution	NULL	NULL	NULL	NULL	gw60_molcell_12_1_147_s_188	12887900	(A) Arp8 preferentially binds to H3 and H4 in solution.	bind
6851	1	2573	7	10	NULL	0	NULL	Arp8	GP		binds		preferentially			H3	GP				NULL	in solution	NULL	NULL	NULL	NULL	gw60_molcell_12_1_147_s_188	12887900	(A) Arp8 preferentially binds to H3 and H4 in solution.	bind
6852	2	2573	7	10	NULL	0	NULL	Arp8	GP		binds		preferentially			H4	GP				NULL	in solution	NULL	NULL	NULL	NULL	gw60_molcell_12_1_147_s_188	12887900	(A) Arp8 preferentially binds to H3 and H4 in solution.	bind
5995	1	2574	6	10	NULL	0	NULL	G	GP	purified	bind					Csk	GP	purified			NULL		NULL	NULL	NULL	NULL	gw60_devcell_2_6_733_s_197	12062086	(A) As shown by anti-Csk Western blot, purified G   bound to Ni-NTA beads pulled down purified Csk, but not boiled Csk. (B) Coimmunoprecipitation experiments with NG108 cell extract showed that anti-Csk antibody precipitated G   bound to Csk after stimulation of mAChR with carbachol.	bind
5996	2	2574	6	10	NULL	0	NULL	G	GP	purified	does not bind					Csk	GP	boiled			NULL		NULL	NULL	NULL	NULL	gw60_devcell_2_6_733_s_197	12062086	(A) As shown by anti-Csk Western blot, purified G   bound to Ni-NTA beads pulled down purified Csk, but not boiled Csk. (B) Coimmunoprecipitation experiments with NG108 cell extract showed that anti-Csk antibody precipitated G   bound to Csk after stimulation of mAChR with carbachol.	bind
5997	3	2574	6	10	NULL	0	NULL	G	GP		bind					Csk	GP				NULL	NG108 cell extract	NULL	NULL	NULL	NULL	gw60_devcell_2_6_733_s_197	12062086	(A) As shown by anti-Csk Western blot, purified G   bound to Ni-NTA beads pulled down purified Csk, but not boiled Csk. (B) Coimmunoprecipitation experiments with NG108 cell extract showed that anti-Csk antibody precipitated G   bound to Csk after stimulation of mAChR with carbachol.	bind
5998	4	2574	6	10	NULL	0	NULL	carbachol	Chemical		stimulates					mAChR	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_2_6_733_s_197	12062086	(A) As shown by anti-Csk Western blot, purified G   bound to Ni-NTA beads pulled down purified Csk, but not boiled Csk. (B) Coimmunoprecipitation experiments with NG108 cell extract showed that anti-Csk antibody precipitated G   bound to Csk after stimulation of mAChR with carbachol.	bind
5999	5	2574	6	10	NULL	0	NULL	statement 3	Process		occurs after					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_devcell_2_6_733_s_197	12062086	(A) As shown by anti-Csk Western blot, purified G   bound to Ni-NTA beads pulled down purified Csk, but not boiled Csk. (B) Coimmunoprecipitation experiments with NG108 cell extract showed that anti-Csk antibody precipitated G   bound to Csk after stimulation of mAChR with carbachol.	bind
6853	1	2574	7	10	NULL	0	NULL	G	GP	purified	binds					Csk	GP	purified			NULL		NULL	NULL	NULL	NULL	gw60_devcell_2_6_733_s_197	12062086	(A) As shown by anti-Csk Western blot, purified G   bound to Ni-NTA beads pulled down purified Csk, but not boiled Csk. (B) Coimmunoprecipitation experiments with NG108 cell extract showed that anti-Csk antibody precipitated G   bound to Csk after stimulation of mAChR with carbachol.	bind
6854	2	2574	7	10	NULL	0	NULL	G	GP	purified	does not bind					Csk	GP	boiled			NULL		NULL	NULL	NULL	NULL	gw60_devcell_2_6_733_s_197	12062086	(A) As shown by anti-Csk Western blot, purified G   bound to Ni-NTA beads pulled down purified Csk, but not boiled Csk. (B) Coimmunoprecipitation experiments with NG108 cell extract showed that anti-Csk antibody precipitated G   bound to Csk after stimulation of mAChR with carbachol.	bind
6855	3	2574	7	10	NULL	0	NULL	G	GP		binds					Csk	GP				NULL	NG108 cell extract 	NULL	NULL	NULL	NULL	gw60_devcell_2_6_733_s_197	12062086	(A) As shown by anti-Csk Western blot, purified G   bound to Ni-NTA beads pulled down purified Csk, but not boiled Csk. (B) Coimmunoprecipitation experiments with NG108 cell extract showed that anti-Csk antibody precipitated G   bound to Csk after stimulation of mAChR with carbachol.	bind
6856	4	2574	7	10	NULL	0	NULL	carbachol 	Chemical		stimulate					mAChR	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_2_6_733_s_197	12062086	(A) As shown by anti-Csk Western blot, purified G   bound to Ni-NTA beads pulled down purified Csk, but not boiled Csk. (B) Coimmunoprecipitation experiments with NG108 cell extract showed that anti-Csk antibody precipitated G   bound to Csk after stimulation of mAChR with carbachol.	bind
6857	5	2574	7	10	NULL	0	NULL	statement 3	Process		occurs after					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_devcell_2_6_733_s_197	12062086	(A) As shown by anti-Csk Western blot, purified G   bound to Ni-NTA beads pulled down purified Csk, but not boiled Csk. (B) Coimmunoprecipitation experiments with NG108 cell extract showed that anti-Csk antibody precipitated G   bound to Csk after stimulation of mAChR with carbachol.	bind
6000	1	2575	6	10	NULL	0	NULL	SBP	GP		bind					glycolipid	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_43_42050_s_70	12917406	(a) Assay for Binding Activity of the SBP Binding of the SBP to Glycolipids --	bind
6861	1	2575	7	10	NULL	0	NULL	SBP	GP		binds to					Glycolipids	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_43_42050_s_70	12917406	(a) Assay for Binding Activity of the SBP Binding of the SBP to Glycolipids --	bind
6001	1	2576	6	10	NULL	0	NULL	GST-MyoD 	GP		bind					MEF-1 oligodeoxynucleotide	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_1074_s_273	9448005	(A) Assays involving the binding of GST-MyoD fusion protein to the MEF-1 oligodeoxynucleotide.	bind
46363	2	2576	6	10	NULL	0	NULL	GST-MyoD	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_1074_s_273	9448005	(A) Assays involving the binding of GST-MyoD fusion protein to the MEF-1 oligodeoxynucleotide.	bind
6862	1	2576	7	10	NULL	0	NULL	GST-MyoD	GP		binds					MEF-1oligodeoxynucleotide	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_1074_s_273	9448005	(A) Assays involving the binding of GST-MyoD fusion protein to the MEF-1 oligodeoxynucleotide.	bind
46364	2	2576	7	10	NULL	0	NULL	GST-MyoD	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_1074_s_273	9448005	(A) Assays involving the binding of GST-MyoD fusion protein to the MEF-1 oligodeoxynucleotide.	bind
6002	1	2577	6	10	NULL	0	NULL	GAPDH	GP		associate					lysosomes	CellComponent	intact 			NULL	untreated fed rats, 48-h starved rats (Strv) or fed rats treated with paraquat (PQ)	NULL	NULL	NULL	NULL	gw70_molbiolcell_15_11_4829_s_197	15331765	(A) Association and binding of GAPDH  and RNase A to intact lysosomes from untreated fed rats, 48-h starved rats (Strv)  or fed rats treated with paraquat (PQ).	bind
6003	2	2577	6	10	NULL	0	NULL	GAPDH	GP		bind					lysosomes	CellComponent	intact 			NULL	untreated fed rats, 48-h starved rats (Strv) or fed rats treated with paraquat (PQ)	NULL	NULL	NULL	NULL	gw70_molbiolcell_15_11_4829_s_197	15331765	(A) Association and binding of GAPDH  and RNase A to intact lysosomes from untreated fed rats, 48-h starved rats (Strv)  or fed rats treated with paraquat (PQ).	bind
6004	3	2577	6	10	NULL	0	NULL	RNase A	GP		bind					 lysosomes	CellComponent	intact			NULL	untreated fed rats, 48-h starved rats (Strv) or fed rats treated with paraquat (PQ)	NULL	NULL	NULL	NULL	gw70_molbiolcell_15_11_4829_s_197	15331765	(A) Association and binding of GAPDH  and RNase A to intact lysosomes from untreated fed rats, 48-h starved rats (Strv)  or fed rats treated with paraquat (PQ).	bind
6005	4	2577	6	10	NULL	0	NULL	RNase A	GP		associate					lysosomes	CellComponent	intact			NULL	untreated fed rats, 48-h starved rats (Strv) or fed rats treated with paraquat (PQ)	NULL	NULL	NULL	NULL	gw70_molbiolcell_15_11_4829_s_197	15331765	(A) Association and binding of GAPDH  and RNase A to intact lysosomes from untreated fed rats, 48-h starved rats (Strv)  or fed rats treated with paraquat (PQ).	bind
6863	1	2577	7	10	NULL	0	NULL	RNaseA	GP		binds					lysosomes	CellComponent	intact;;rat			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_11_4829_s_197	15331765	(A) Association and binding of GAPDH  and RNase A to intact lysosomes from untreated fed rats, 48-h starved rats (Strv)  or fed rats treated with paraquat (PQ).	bind
6864	2	2577	7	10	NULL	0	NULL	GAPDH	GP		binds					lysosomes	CellComponent	intact;;rat			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_11_4829_s_197	15331765	(A) Association and binding of GAPDH  and RNase A to intact lysosomes from untreated fed rats, 48-h starved rats (Strv)  or fed rats treated with paraquat (PQ).	bind
6006	1	2578	6	10	NULL	0	NULL	Ast*	GP		bind					CRF-R1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_288_2_729_s_60	9918582	(A) Ast* or (B) Ucn* bound to CRF-R1 by astressin ( ), r/hCRF ( ) and Ucn ( ).	bind
6007	2	2578	6	10	NULL	0	NULL	Ucn*	GP		bind					CRF-R1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_288_2_729_s_60	9918582	(A) Ast* or (B) Ucn* bound to CRF-R1 by astressin ( ), r/hCRF ( ) and Ucn ( ).	bind
6008	3	2578	6	10	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_288_2_729_s_60	9918582	(A) Ast* or (B) Ucn* bound to CRF-R1 by astressin ( ), r/hCRF ( ) and Ucn ( ).	bind
6865	1	2578	7	10	NULL	0	NULL	Ast*	GP		binds					CRF-R1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_288_2_729_s_60	9918582	(A) Ast* or (B) Ucn* bound to CRF-R1 by astressin ( ), r/hCRF ( ) and Ucn ( ).	bind
6866	2	2578	7	10	NULL	0	NULL	Ucn*	GP		binds					CRF-R1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_288_2_729_s_60	9918582	(A) Ast* or (B) Ucn* bound to CRF-R1 by astressin ( ), r/hCRF ( ) and Ucn ( ).	bind
6867	3	2578	7	10	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_288_2_729_s_60	9918582	(A) Ast* or (B) Ucn* bound to CRF-R1 by astressin ( ), r/hCRF ( ) and Ucn ( ).	bind
6009	1	2579	6	10	NULL	0	NULL	ATM	GP		phosphorylates					p53	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_1_s_360	16267266	(a) ATM phosphorylates  p53; this phosphorylation blocks the binding of p53 to Mdm2, thereby preventing rapid  MdM2-induced p53 degradation.	bind
6010	2	2579	6	10	NULL	0	NULL	p53	GP		bind					Mdm2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_1_s_360	16267266	(a) ATM phosphorylates  p53; this phosphorylation blocks the binding of p53 to Mdm2, thereby preventing rapid  MdM2-induced p53 degradation.	bind
6011	3	2579	6	10	NULL	0	NULL	statement 1	Process		blocks					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_1_s_360	16267266	(a) ATM phosphorylates  p53; this phosphorylation blocks the binding of p53 to Mdm2, thereby preventing rapid  MdM2-induced p53 degradation.	bind
6012	4	2579	6	10	NULL	0	NULL	MdM2	GP		induces					p53	GP	degradation of			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_1_s_360	16267266	(a) ATM phosphorylates  p53; this phosphorylation blocks the binding of p53 to Mdm2, thereby preventing rapid  MdM2-induced p53 degradation.	bind
6013	5	2579	6	10	NULL	0	NULL	statement 3	Process		prevents					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_1_s_360	16267266	(a) ATM phosphorylates  p53; this phosphorylation blocks the binding of p53 to Mdm2, thereby preventing rapid  MdM2-induced p53 degradation.	bind
6868	1	2579	7	10	NULL	0	NULL	ATM	GP		phosphorylates					p53	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_1_s_360	16267266	(a) ATM phosphorylates  p53; this phosphorylation blocks the binding of p53 to Mdm2, thereby preventing rapid  MdM2-induced p53 degradation.	bind
6869	2	2579	7	10	NULL	0	NULL	p53	GP		binds					Mdm2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_1_s_360	16267266	(a) ATM phosphorylates  p53; this phosphorylation blocks the binding of p53 to Mdm2, thereby preventing rapid  MdM2-induced p53 degradation.	bind
6870	3	2579	7	10	NULL	0	NULL	statement 1	Process		blocks					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_1_s_360	16267266	(a) ATM phosphorylates  p53; this phosphorylation blocks the binding of p53 to Mdm2, thereby preventing rapid  MdM2-induced p53 degradation.	bind
6871	4	2579	7	10	NULL	0	NULL	MdM2	GP		induce					p53	GP	degradation of			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_1_s_360	16267266	(a) ATM phosphorylates  p53; this phosphorylation blocks the binding of p53 to Mdm2, thereby preventing rapid  MdM2-induced p53 degradation.	bind
7913	5	2579	7	10	NULL	0	NULL	statement 3	Process		prevents					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_1_s_360	16267266	(a) ATM phosphorylates  p53; this phosphorylation blocks the binding of p53 to Mdm2, thereby preventing rapid  MdM2-induced p53 degradation.	bind
6014	1	2581	6	10	NULL	0	NULL	ATP	Chemical		bind					erbB2	GP		active site		NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_307_2_267_s_51	12859950	(A) ATP bound to the active site of erbB2.	bind
6872	1	2581	7	10	NULL	0	NULL	ATP	Chemical		bind					erbB2	GP		active site		NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_307_2_267_s_51	12859950	(A) ATP bound to the active site of erbB2.	bind
6015	1	2582	6	10	NULL	0	NULL	PKA	GP		phosphorylates					RyR1	GP				NULL	skeletal muscle of sham-operated (control) and HF rats	NULL	NULL	NULL	NULL	gw70_cellbiol_160_6_919_s_164	12629052	(A) Autoradiogram showing PKA back phosphorylation of RyR1 from skeletal muscle of  sham-operated (control) and HF rats, bar graph shows relative PKA phosphorylation  of RyR1 (expressed as inverse of back phosphorylation as previously described [ ]).	bind
6873	1	2582	7	10	NULL	0	NULL	PKA	GP		phosphorylate					RyR1	GP				NULL	from skeletal muscle of sham-operated and HF rats	NULL	NULL	NULL	NULL	gw70_cellbiol_160_6_919_s_164	12629052	(A) Autoradiogram showing PKA back phosphorylation of RyR1 from skeletal muscle of  sham-operated (control) and HF rats, bar graph shows relative PKA phosphorylation  of RyR1 (expressed as inverse of back phosphorylation as previously described [ ]).	bind
6016	1	2586	6	10	NULL	0	NULL	Bax	GP		bind			BH3 domain		Bcl-2 family members	GP	pro-apoptotic factor			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_currbiol_7_12_913_s_95	9382837	(a) BH3 domains from Bax and Bak can bind to pro-apoptotic and anti-apoptotic Bcl-2 family members  in vitro.	bind
6017	2	2586	6	10	NULL	0	NULL	bak	GP		bind			BH3 domain		Bcl-2 family members	GP	pro-apoptotic factor			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_currbiol_7_12_913_s_95	9382837	(a) BH3 domains from Bax and Bak can bind to pro-apoptotic and anti-apoptotic Bcl-2 family members  in vitro.	bind
7871	3	2586	6	10	NULL	0	NULL	Bax	GP		bind			BH3 domain		Bcl-2 family members	GP	anti-apoptotic			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_currbiol_7_12_913_s_95	9382837	(a) BH3 domains from Bax and Bak can bind to pro-apoptotic and anti-apoptotic Bcl-2 family members  in vitro.	bind
7872	4	2586	6	10	NULL	0	NULL	Bak	GP		bind			BH3 domain		Bcl-2 family members	GP	anti-apoptotic			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_currbiol_7_12_913_s_95	9382837	(a) BH3 domains from Bax and Bak can bind to pro-apoptotic and anti-apoptotic Bcl-2 family members  in vitro.	bind
6886	1	2586	7	10	NULL	0	NULL	Bax	GP		bind			BH3 domain		Bcl-2 family members	GP	pro-apoptotic			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_currbiol_7_12_913_s_95	9382837	(a) BH3 domains from Bax and Bak can bind to pro-apoptotic and anti-apoptotic Bcl-2 family members  in vitro.	bind
6887	2	2586	7	10	NULL	0	NULL	Bak	GP		bind			BH3 domain		Bcl-2 family members	GP	pro-apoptotic			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_currbiol_7_12_913_s_95	9382837	(a) BH3 domains from Bax and Bak can bind to pro-apoptotic and anti-apoptotic Bcl-2 family members  in vitro.	bind
6888	3	2586	7	10	NULL	0	NULL	Bax	GP		bind			BH3 domain		Bcl-2 family members	GP	anti-apoptotic			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_currbiol_7_12_913_s_95	9382837	(a) BH3 domains from Bax and Bak can bind to pro-apoptotic and anti-apoptotic Bcl-2 family members  in vitro.	bind
6889	4	2586	7	10	NULL	0	NULL	Bak	GP		bind			BH3 domain		Bcl-2 family members	GP	anti-apoptotic			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_currbiol_7_12_913_s_95	9382837	(a) BH3 domains from Bax and Bak can bind to pro-apoptotic and anti-apoptotic Bcl-2 family members  in vitro.	bind
6018	1	2588	6	10	NULL	0	NULL	GCK	GP	endogenous	bind					TRAF6	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_9165_s_282	15456887	(A) Binding  of endogenous GCK to TRAF6.	bind
6890	1	2588	7	10	NULL	0	NULL	GCK	GP	endogenous	binds					TRAF6	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_9165_s_282	15456887	(A) Binding  of endogenous GCK to TRAF6.	bind
6019	1	2589	6	10	NULL	0	NULL	Tac1p-GST	GP		bind									GRE	NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_3_6_1639_s_122	15590837	(A) Binding  saturation of the DRE by Tac1p-GST.	bind
6891	1	2589	7	10	NULL	0	NULL	Tac1p-GST	GP		binds									DRE	NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_3_6_1639_s_122	15590837	(A) Binding  saturation of the DRE by Tac1p-GST.	bind
7873	1	2590	6	10	NULL	0	NULL	Paip1	GP		bind					PABP	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3769_s_403	11997512	(A) binding activity of PABP ( 6,  24) and Paip1 interacts strongly with this region, additional experiments will be necessary to determine whether Paip1 binding to PABP affects the poly	bind
6892	1	2590	7	10	NULL	0	NULL	Paip1	GP		binds					PABP	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3769_s_403	11997512	(A) binding activity of PABP ( 6,  24) and Paip1 interacts strongly with this region, additional experiments will be necessary to determine whether Paip1 binding to PABP affects the poly	bind
6020	1	2593	6	10	NULL	0	NULL	eIF4F	GP		bind					m7G cap	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_23_17740_s_17	10748132	(A) binding affinity of PABP and the m7G-cap binding affinity of eIF4F and eIF-iso4F ( 5,  6).	bind
6021	2	2593	6	10	NULL	0	NULL	eIF-iso4F	GP		bind					m7G cap	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_23_17740_s_17	10748132	(A) binding affinity of PABP and the m7G-cap binding affinity of eIF4F and eIF-iso4F ( 5,  6).	bind
6895	3	2593	7	10	NULL	0	NULL	m7G-cap	NucleicAcid		binds					eIF4F	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_23_17740_s_17	10748132	(A) binding affinity of PABP and the m7G-cap binding affinity of eIF4F and eIF-iso4F ( 5,  6).	bind
6896	4	2593	7	10	NULL	0	NULL	m7G-cap	NucleicAcid		binds					eIF-iso4F	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_23_17740_s_17	10748132	(A) binding affinity of PABP and the m7G-cap binding affinity of eIF4F and eIF-iso4F ( 5,  6).	bind
6022	1	2595	6	10	NULL	0	NULL	peptide	GP	synthetic	bind					MAb 15F3-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclinmicrobiol_39_3_977_s_108	11230414	(A) Binding assay of synthetic peptide with MAb 15F3-1.	bind
6897	1	2595	7	10	NULL	0	NULL	peptide	GP	synthetic	binds					MAb 15F3-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclinmicrobiol_39_3_977_s_108	11230414	(A) Binding assay of synthetic peptide with MAb 15F3-1.	bind
6023	1	2596	6	10	NULL	0	NULL	C5	GP	free	bind					p16	GP	S-tagged			NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_3_421_s_176	9660926	(A) Binding between free C5 and S-tagged p16.	bind
6898	1	2596	7	10	NULL	0	NULL	C5	GP	free	binds					p16	GP	S-tagged			NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_3_421_s_176	9660926	(A) Binding between free C5 and S-tagged p16.	bind
6024	1	2597	6	10	NULL	0	NULL	Nef	GP		bind					V1H	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_13_6_2045_s_156	12058068	(A) Binding between Nef and V1H, beta1, and beta2 using the yeast two hybrid liquid assay.	bind
6025	2	2597	6	10	NULL	0	NULL	Nef	GP		bind								beta2		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_13_6_2045_s_156	12058068	(A) Binding between Nef and V1H, beta1, and beta2 using the yeast two hybrid liquid assay.	bind
7874	3	2597	6	10	NULL	0	NULL	Nef	GP		bind								beta 1		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_13_6_2045_s_156	12058068	(A) Binding between Nef and V1H, beta1, and beta2 using the yeast two hybrid liquid assay.	bind
6899	1	2597	7	10	NULL	0	NULL	Nef	GP		binds					V1H	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_13_6_2045_s_156	12058068	(A) Binding between Nef and V1H, beta1, and beta2 using the yeast two hybrid liquid assay.	bind
6900	2	2597	7	10	NULL	0	NULL	Nef	GP		binds								beta1		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_13_6_2045_s_156	12058068	(A) Binding between Nef and V1H, beta1, and beta2 using the yeast two hybrid liquid assay.	bind
7936	3	2597	7	10	NULL	0	NULL	Nef 	GP		binds								beta2		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_13_6_2045_s_156	12058068	(A) Binding between Nef and V1H, beta1, and beta2 using the yeast two hybrid liquid assay.	bind
6026	1	2599	6	10	NULL	0	NULL	BAZF	GP		bind			148-319d27		Bcl6	GP		1-520		NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_303_2_600_s_115	12659862	(A) Binding of  BAZF(148-319d27) deleted with the 27 aa including the conserved 17 aa to Bcl6(1-520)  by the mammalian two-hybrid assay.	bind
6901	1	2599	7	10	NULL	0	NULL	BAZF	GP		binds			148-319d27		Bcl6	GP		1-520		NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_303_2_600_s_115	12659862	(A) Binding of  BAZF(148-319d27) deleted with the 27 aa including the conserved 17 aa to Bcl6(1-520)  by the mammalian two-hybrid assay.	bind
6027	1	2600	6	10	NULL	0	NULL	plectin	GP		bind			ABD		plectin 1C	GP		ABD		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
6028	2	2600	6	10	NULL	0	NULL	plectin	GP		bind			ABD					beta4		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
6029	3	2600	6	10	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
6030	4	2600	6	10	NULL	0	NULL	dystonin	GP		bind			ABD		plectin 1C	GP		ABD		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
6031	5	2600	6	10	NULL	0	NULL	dystonin	GP		bind			ABD					beta4		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
6032	6	2600	6	10	NULL	0	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
6033	7	2600	6	10	NULL	0	NULL	dystrophin	GP		bind			ABD		plectin 1C	GP		ABD		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
6034	8	2600	6	10	NULL	0	NULL	dystrophin	GP		bind			ABD					beta4		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
6035	9	2600	6	10	NULL	0	NULL	statement 7	Process		is an alternative to					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
6036	10	2600	6	10	NULL	0	NULL	alpha-actinin	GP		bind			ABD		plectin 1C	GP		ABD		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
6037	11	2600	6	10	NULL	0	NULL	alpha-actinin	GP		bind			ABD					beta4		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
6038	12	2600	6	10	NULL	0	NULL	statement 10	Process		is an alternative to					statement 11	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
6039	13	2600	6	10	NULL	0	NULL	utrophin	GP		bind			ABD		plectin 1C	GP		ABD		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
6040	14	2600	6	10	NULL	0	NULL	utrophin	GP		bind			ABD					beta4		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
6041	15	2600	6	10	NULL	0	NULL	statement 13	Process		is an alternative to					statement 14	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
6042	16	2600	6	10	NULL	0	NULL	filamin	GP		bind			ABD		plectin 1C	GP		ABD		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
6043	17	2600	6	10	NULL	0	NULL	filamin	GP		bind			ABD					beta4		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
6044	18	2600	6	10	NULL	0	NULL	statement 16	Process		is an alternative to					statement 17	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
7067	1	2600	7	10	NULL	0	NULL	plectin	GP		binds			ABD					beta4		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
7068	2	2600	7	10	NULL	0	NULL	plectin	GP		binds			ABD		plectin-1C	GP		ABD		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
7069	3	2600	7	10	NULL	0	NULL	dystonin	GP		binds			ABD					beta4		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
7070	4	2600	7	10	NULL	0	NULL	dystonin	GP		binds			ABD		plectin-1C	GP		ABD		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
7071	5	2600	7	10	NULL	0	NULL	dystrophin	GP		binds			ABD					beta4		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
7072	6	2600	7	10	NULL	0	NULL	dystrophin	GP		binds			ABD		plectin-1C	GP		ABD		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
7073	7	2600	7	10	NULL	0	NULL	alpha-actinin	GP		binds			ABD					beta4		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
7074	8	2600	7	10	NULL	0	NULL	alpha-actinin	GP		binds			ABD		plectin-1C	GP		ABD		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
7075	9	2600	7	10	NULL	0	NULL	utrophin	GP		binds			ABD					beta4		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
7076	10	2600	7	10	NULL	0	NULL	utrophin	GP		binds			ABD		plectin-1C	GP		ABD		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
7077	11	2600	7	10	NULL	0	NULL	filamin	GP		binds			ABD					beta4		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
7078	12	2600	7	10	NULL	0	NULL	filamin	GP		binds			ABD		plectin-1C	GP		ABD		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
46591	13	2600	7	10	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
46592	14	2600	7	10	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
46593	15	2600	7	10	NULL	0	NULL	statement 5	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
46594	16	2600	7	10	NULL	0	NULL	statement 7	Process		is an alternative to					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
46595	17	2600	7	10	NULL	0	NULL	statement 9	Process		is an alternative to					statement 10	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
46596	18	2600	7	10	NULL	0	NULL	statement 11	Process		is an alternative to					statement 12	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_10_4039_s_68	14517317	(A) Binding of ABDs of plectin, dystonin, dystrophin,  alpha-actinin, utrophin and filamin to either beta4 or the plectin-1C ABD.	bind
4576	1	2601	5	10	NULL	0	NULL	ActA peptide	GP		bind			DFPPPPTDEEL		Mena	GP		EVH1 domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_97_4_471_s_61	10338211	(A) Binding of ActA peptide (DFPPPPTDEEL) to the Mena EVH1 domain, measured using  a fluorescence perturbation assay.	bind
7079	1	2601	7	10	NULL	0	NULL	ActA peptide	GP		binds			DFPPPPTDEEL		Mena	GP		EVH1		NULL		NULL	NULL	NULL	NULL	gw60_cell_97_4_471_s_61	10338211	(A) Binding of ActA peptide (DFPPPPTDEEL) to the Mena EVH1 domain, measured using  a fluorescence perturbation assay.	bind
4578	1	2602	5	10	NULL	0	NULL	AIM2	GP		bind					GST-p202	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_474_1_38_s_145	10828447	(a) Binding of AIM2 to GST-p202.	bind
7080	1	2602	7	10	NULL	0	NULL	 AIM2	GP		binds					GST-p202	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_474_1_38_s_145	10828447	(a) Binding of AIM2 to GST-p202.	bind
4579	1	2603	5	10	NULL	0	NULL	AP-1	GP		bind					GST-Nef	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_22_1235_s_70	9811606	(a) Binding of AP-1 to GST-Nef fusion proteins.	bind
7081	1	2603	7	10	NULL	0	NULL	AP-1	GP		binds					GST-Nef	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_22_1235_s_70	9811606	(a) Binding of AP-1 to GST-Nef fusion proteins.	bind
4581	1	2605	5	10	NULL	0	NULL	B-cell nuclear extract proteins	GP		bind					mb-1	GP			distal region	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_24_8539_s_236	12446773	(A) Binding of B-cell nuclear extract proteins to the  mb-1 distal region is specifically inhibited by wild type, but not mutated  mb-1 promoter sequences.	bind
4582	2	2605	5	10	NULL	0	NULL	mb-1	GP	wild-type	inhibit		specifically		promoter	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_24_8539_s_236	12446773	(A) Binding of B-cell nuclear extract proteins to the  mb-1 distal region is specifically inhibited by wild type, but not mutated  mb-1 promoter sequences.	bind
4583	3	2605	5	10	NULL	0	NULL	mb-1	GP	mutant	does not inhibit				promoter sequences	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_24_8539_s_236	12446773	(A) Binding of B-cell nuclear extract proteins to the  mb-1 distal region is specifically inhibited by wild type, but not mutated  mb-1 promoter sequences.	bind
7083	1	2605	7	10	NULL	0	NULL	B-cell nuclear extract proteins	GP		binds 					 mb-1	GP			distal region	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_24_8539_s_236	12446773	(A) Binding of B-cell nuclear extract proteins to the  mb-1 distal region is specifically inhibited by wild type, but not mutated  mb-1 promoter sequences.	bind
7084	2	2605	7	10	NULL	0	NULL	statement 1	Process		 inhibited by		specifically			mb-1	GP	wild type		promoter sequences	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_24_8539_s_236	12446773	(A) Binding of B-cell nuclear extract proteins to the  mb-1 distal region is specifically inhibited by wild type, but not mutated  mb-1 promoter sequences.	bind
7085	3	2605	7	10	NULL	0	NULL	statement 1	Process		is not inhibited by					mb-1	GP	mutated		promoter sequences	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_24_8539_s_236	12446773	(A) Binding of B-cell nuclear extract proteins to the  mb-1 distal region is specifically inhibited by wild type, but not mutated  mb-1 promoter sequences.	bind
4584	1	2606	5	10	NULL	0	NULL	c-Src	GP		bind					mDia1	GP	active			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_18_6844_s_87	16943426	(A) Binding of c-Src by active mDia1.	bind
7086	1	2606	7	10	NULL	0	NULL	c-Src	GP		binds					mDia1	GP	active			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_18_6844_s_87	16943426	(A) Binding of c-Src by active mDia1.	bind
4585	1	2607	5	10	NULL	0	NULL	C/EBP	GP		bind									C/EBP-binding element	NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_293_3_907_s_102	12051744	(A) Binding of C/EBP  and C/EBP  to a C/EBP-binding element is increased after treatment with glucocorticoids.	bind
4586	2	2607	5	10	NULL	0	NULL	glucocorticoids	Chemical	treatment	increase					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_293_3_907_s_102	12051744	(A) Binding of C/EBP  and C/EBP  to a C/EBP-binding element is increased after treatment with glucocorticoids.	bind
7087	1	2607	7	10	NULL	0	NULL	C/EBP 	GP		binds to									C/EBP-binding element	NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_293_3_907_s_102	12051744	(A) Binding of C/EBP  and C/EBP  to a C/EBP-binding element is increased after treatment with glucocorticoids.	bind
7088	2	2607	7	10	NULL	0	NULL	glucocorticoids	Chemical	treatment with	increases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_293_3_907_s_102	12051744	(A) Binding of C/EBP  and C/EBP  to a C/EBP-binding element is increased after treatment with glucocorticoids.	bind
4587	1	2608	5	10	NULL	0	NULL	c95A0 	GP		bind			c21		dystroglycan	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_16_4_755_s_158	8607994	(A) Binding of c95A0 c21 and c95A4 c21 to  -dystroglycan.	bind
4588	2	2608	5	10	NULL	0	NULL	c95A4 	GP		bind			c21		dystroglycan	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_16_4_755_s_158	8607994	(A) Binding of c95A0 c21 and c95A4 c21 to  -dystroglycan.	bind
7089	1	2608	7	10	NULL	0	NULL	c95A0	GP		binds			c21		dystroglycan	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_16_4_755_s_158	8607994	(A) Binding of c95A0 c21 and c95A4 c21 to  -dystroglycan.	bind
7090	2	2608	7	10	NULL	0	NULL	 c95A4 	GP		binds 			c21		dystroglycan	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_16_4_755_s_158	8607994	(A) Binding of c95A0 c21 and c95A4 c21 to  -dystroglycan.	bind
4678	1	2609	5	10	NULL	0	NULL	c95A0	GP		lack			c21					C-terminal 21 kDa		NULL		NULL	NULL	NULL	NULL	gw60_neuron_16_4_755_s_193	8607994	(A) Binding of c95A0 c21 and c95A4 c21, lacking the most C-terminal 21 kDa, to chick muscle cells.	bind
4683	2	2609	5	10	NULL	0	NULL	statement 1	GP		bind					muscle cells	Cell	chick			NULL		NULL	NULL	NULL	NULL	gw60_neuron_16_4_755_s_193	8607994	(A) Binding of c95A0 c21 and c95A4 c21, lacking the most C-terminal 21 kDa, to chick muscle cells.	bind
4684	3	2609	5	10	NULL	0	NULL	c95A4	GP		lack			c21					C-terminal 21 kDa		NULL		NULL	NULL	NULL	NULL	gw60_neuron_16_4_755_s_193	8607994	(A) Binding of c95A0 c21 and c95A4 c21, lacking the most C-terminal 21 kDa, to chick muscle cells.	bind
4686	4	2609	5	10	NULL	0	NULL	statement 1	GP		bind					muscle cells	Cell	chick			NULL		NULL	NULL	NULL	NULL	gw60_neuron_16_4_755_s_193	8607994	(A) Binding of c95A0 c21 and c95A4 c21, lacking the most C-terminal 21 kDa, to chick muscle cells.	bind
7091	1	2609	7	10	NULL	0	NULL	c95A0	GP		binds			c21		muscle cells	Cell	chick			NULL		NULL	NULL	NULL	NULL	gw60_neuron_16_4_755_s_193	8607994	(A) Binding of c95A0 c21 and c95A4 c21, lacking the most C-terminal 21 kDa, to chick muscle cells.	bind
7092	2	2609	7	10	NULL	0	NULL	c95A4	GP		binds			c21		muscle cells	Cell	chick			NULL		NULL	NULL	NULL	NULL	gw60_neuron_16_4_755_s_193	8607994	(A) Binding of c95A0 c21 and c95A4 c21, lacking the most C-terminal 21 kDa, to chick muscle cells.	bind
7093	3	2609	7	10	NULL	0	NULL	c95A0	GP		lacks								C-terminal 21 kDa		NULL		NULL	NULL	NULL	NULL	gw60_neuron_16_4_755_s_193	8607994	(A) Binding of c95A0 c21 and c95A4 c21, lacking the most C-terminal 21 kDa, to chick muscle cells.	bind
7094	4	2609	7	10	NULL	0	NULL	c95A4	GP		lacks								C-terminal 21 kDa		NULL		NULL	NULL	NULL	NULL	gw60_neuron_16_4_755_s_193	8607994	(A) Binding of c95A0 c21 and c95A4 c21, lacking the most C-terminal 21 kDa, to chick muscle cells.	bind
4689	1	2610	5	10	NULL	0	NULL	CCR1 antisera			bind					CCR1 receptor	GP	transfectants			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_2_112_s_49	9024623	(a) Binding of CCR1 antisera to CCR1 receptor transfectants.	bind
7095	1	2610	7	10	NULL	0	NULL	CCR1 antisera			binds					CCR1 receptor	GP	transfectant			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_2_112_s_49	9024623	(a) Binding of CCR1 antisera to CCR1 receptor transfectants.	bind
4692	1	2611	5	10	NULL	0	NULL	HCP	GP	cellular	bind					p58	GP	phosphotyrosyl peptides			NULL		NULL	NULL	NULL	NULL	gw60_immunity_4_1_77_s_138	8574854	(A) Binding of cellular HCP to p58 phosphotyrosyl peptides.	bind
7096	1	2611	7	10	NULL	0	NULL	HCP	GP	cellular	binds					p58	GP	phosphotyrosyl peptides			NULL		NULL	NULL	NULL	NULL	gw60_immunity_4_1_77_s_138	8574854	(A) Binding of cellular HCP to p58 phosphotyrosyl peptides.	bind
4693	1	2612	5	10	NULL	0	NULL	CIDR1alpha	GP		bind					Igs fragments	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_9_5412_s_162	15322039	(A) Binding of CIDR1alpha to human Igs and Ig fragments.	bind
4694	2	2612	5	10	NULL	0	NULL	CIDR1alpha	GP		bind					Ig fragments	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_9_5412_s_162	15322039	(A) Binding of CIDR1alpha to human Igs and Ig fragments.	bind
7097	1	2612	7	10	NULL	0	NULL	CIDR1alpha	GP		binds					Igs	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_9_5412_s_162	15322039	(A) Binding of CIDR1alpha to human Igs and Ig fragments.	bind
7098	2	2612	7	10	NULL	0	NULL	CIDR1alpha	GP		binds					Ig fragments	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_9_5412_s_162	15322039	(A) Binding of CIDR1alpha to human Igs and Ig fragments.	bind
4698	1	2613	5	10	NULL	0	NULL	CMV gB	GP		bind					DC-SIGN	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_5_653_s_177	12433371	(A) Binding of CMV gB to DC-SIGN.	bind
7099	1	2613	7	10	NULL	0	NULL	CMV gB	GP		binds					DC-SIGN	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_5_653_s_177	12433371	(A) Binding of CMV gB to DC-SIGN.	bind
4948	1	2614	5	10	NULL	0	NULL	EF-G	GP		bind					RC	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_87	12859902	(A) Binding of EF-G and GDP to RC Before and After Release of Peptide from the P-site tRNA with and without fus.	bind
4949	2	2614	5	10	NULL	0	NULL	peptide	AminoAcid		released from					tRNA	NucleicAcid		P-site		NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_87	12859902	(A) Binding of EF-G and GDP to RC Before and After Release of Peptide from the P-site tRNA with and without fus.	bind
4950	3	2614	5	10	NULL	0	NULL	statement 2	Process		occurs with					fus	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_87	12859902	(A) Binding of EF-G and GDP to RC Before and After Release of Peptide from the P-site tRNA with and without fus.	bind
4951	4	2614	5	10	NULL	0	NULL	statement 2	Process		occurs without					fus	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_87	12859902	(A) Binding of EF-G and GDP to RC Before and After Release of Peptide from the P-site tRNA with and without fus.	bind
4952	5	2614	5	10	NULL	0	NULL	statement 1	Process		occurs before					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_87	12859902	(A) Binding of EF-G and GDP to RC Before and After Release of Peptide from the P-site tRNA with and without fus.	bind
4953	6	2614	5	10	NULL	0	NULL	statement 1	Process		occurs after					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_87	12859902	(A) Binding of EF-G and GDP to RC Before and After Release of Peptide from the P-site tRNA with and without fus.	bind
4954	7	2614	5	10	NULL	0	NULL	GDP	Chemical		bind					RC	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_87	12859902	(A) Binding of EF-G and GDP to RC Before and After Release of Peptide from the P-site tRNA with and without fus.	bind
4955	8	2614	5	10	NULL	0	NULL	statement 7	NULL		occurs before	NULL				statement 4	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_87	12859902	(A) Binding of EF-G and GDP to RC Before and After Release of Peptide from the P-site tRNA with and without fus.	bind
4956	9	2614	5	10	NULL	0	NULL	statement 7	NULL		occurs after	NULL				statement 4	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_87	12859902	(A) Binding of EF-G and GDP to RC Before and After Release of Peptide from the P-site tRNA with and without fus.	bind
7100	1	2614	7	10	NULL	0	NULL	EF-G	GP		binds					RC	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_87	12859902	(A) Binding of EF-G and GDP to RC Before and After Release of Peptide from the P-site tRNA with and without fus.	bind
7101	2	2614	7	10	NULL	0	NULL	GDP	Chemical		binds					RC	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_87	12859902	(A) Binding of EF-G and GDP to RC Before and After Release of Peptide from the P-site tRNA with and without fus.	bind
7102	3	2614	7	10	NULL	0	NULL	statement 1	Process		occurs before					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_87	12859902	(A) Binding of EF-G and GDP to RC Before and After Release of Peptide from the P-site tRNA with and without fus.	bind
7103	4	2614	7	10	NULL	0	NULL	statement 1	Process		occurs after					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_87	12859902	(A) Binding of EF-G and GDP to RC Before and After Release of Peptide from the P-site tRNA with and without fus.	bind
7110	5	2614	7	10	NULL	0	NULL	peptide	AminoAcid		release from					tRNA	NucleicAcid		P-site 		NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_87	12859902	(A) Binding of EF-G and GDP to RC Before and After Release of Peptide from the P-site tRNA with and without fus.	bind
7112	6	2614	7	10	NULL	0	NULL	statement 2	Process		occurs before					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_87	12859902	(A) Binding of EF-G and GDP to RC Before and After Release of Peptide from the P-site tRNA with and without fus.	bind
7115	7	2614	7	10	NULL	0	NULL	statement 2	Process		occurs after					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_87	12859902	(A) Binding of EF-G and GDP to RC Before and After Release of Peptide from the P-site tRNA with and without fus.	bind
4707	1	2615	5	10	NULL	0	NULL	M-280 protein A Dynabeads			coated with					2D VCAM-1 - Fc	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_6_1073_s_130	16365170	(A) Binding of either wt or Y991A alpha4beta1-expressing cells to M-280 protein A Dynabeads coated with 2D VCAM-1 - Fc. Relative  bead binding was determined by side scattering analysis.	bind
4709	2	2615	5	10	NULL	0	NULL	alpha4beta1-expressing cells	Cell	wt	bind					statement 1					NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_6_1073_s_130	16365170	(A) Binding of either wt or Y991A alpha4beta1-expressing cells to M-280 protein A Dynabeads coated with 2D VCAM-1 - Fc. Relative  bead binding was determined by side scattering analysis.	bind
4711	3	2615	5	10	NULL	0	NULL	alpha4beta1-expressing cells	Cell		bind			Y991A		statement 1					NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_6_1073_s_130	16365170	(A) Binding of either wt or Y991A alpha4beta1-expressing cells to M-280 protein A Dynabeads coated with 2D VCAM-1 - Fc. Relative  bead binding was determined by side scattering analysis.	bind
4712	4	2615	5	10	NULL	0	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_6_1073_s_130	16365170	(A) Binding of either wt or Y991A alpha4beta1-expressing cells to M-280 protein A Dynabeads coated with 2D VCAM-1 - Fc. Relative  bead binding was determined by side scattering analysis.	bind
7122	1	2615	7	10	NULL	0	NULL	alpha4beta1-expressing cells	Cell	wt	binds					M-280 protein A dynabeads					NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_6_1073_s_130	16365170	(A) Binding of either wt or Y991A alpha4beta1-expressing cells to M-280 protein A Dynabeads coated with 2D VCAM-1 - Fc. Relative  bead binding was determined by side scattering analysis.	bind
7124	2	2615	7	10	NULL	0	NULL	M-280 protein A Dynabeads			is coated with					2D VCAM-1 - Fc	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_6_1073_s_130	16365170	(A) Binding of either wt or Y991A alpha4beta1-expressing cells to M-280 protein A Dynabeads coated with 2D VCAM-1 - Fc. Relative  bead binding was determined by side scattering analysis.	bind
7125	3	2615	7	10	NULL	0	NULL	alpha4beta1-expressing cells	Cell		binds			 Y991A		M-280 protein A dynabeads					NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_6_1073_s_130	16365170	(A) Binding of either wt or Y991A alpha4beta1-expressing cells to M-280 protein A Dynabeads coated with 2D VCAM-1 - Fc. Relative  bead binding was determined by side scattering analysis.	bind
4790	1	2616	5	10	NULL	0	NULL	En2deltaSP	GP		bind									HF1 site	NULL		NULL	NULL	NULL	NULL	gw60_development_130_9_1867_s_84	12642491	(A) Binding of En2deltaSP and Foxa2 to the HF1 site.	bind
4791	2	2616	5	10	NULL	0	NULL	Foxa2	GP		bind									HF1 site	NULL		NULL	NULL	NULL	NULL	gw60_development_130_9_1867_s_84	12642491	(A) Binding of En2deltaSP and Foxa2 to the HF1 site.	bind
7126	1	2616	7	10	NULL	0	NULL	En2deltaSP	GP		binds to									HF1 site	NULL		NULL	NULL	NULL	NULL	gw60_development_130_9_1867_s_84	12642491	(A) Binding of En2deltaSP and Foxa2 to the HF1 site.	bind
7127	2	2616	7	10	NULL	0	NULL	Foxa2	GP		binds to									HF1 site	NULL		NULL	NULL	NULL	NULL	gw60_development_130_9_1867_s_84	12642491	(A) Binding of En2deltaSP and Foxa2 to the HF1 site.	bind
4807	1	2617	5	10	NULL	0	NULL	FGF10	GP		bind					HSPG	GP				NULL	lung epithelial cells	NULL	NULL	NULL	NULL	gw70_devbiol_258_1_185_s_123	12781692	(A) Binding of FGF10 to HSPG is increased when compared with FGF7 in confluent  20-3 lung epithelial cells; however, binding to FGFR2 is similar for both FGFs (see  Materials and methods).	bind
4808	2	2617	5	10	NULL	0	NULL	FGF7	GP		bind					HSPG	GP				NULL	lung epithelial cells	NULL	NULL	NULL	NULL	gw70_devbiol_258_1_185_s_123	12781692	(A) Binding of FGF10 to HSPG is increased when compared with FGF7 in confluent  20-3 lung epithelial cells; however, binding to FGFR2 is similar for both FGFs (see  Materials and methods).	bind
4810	3	2617	5	10	NULL	0	NULL	FGF10	GP		bind					FGFR2	GP				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_258_1_185_s_123	12781692	(A) Binding of FGF10 to HSPG is increased when compared with FGF7 in confluent  20-3 lung epithelial cells; however, binding to FGFR2 is similar for both FGFs (see  Materials and methods).	bind
4811	4	2617	5	10	NULL	0	NULL	FGF7	GP		bind					FGFR2	GP				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_258_1_185_s_123	12781692	(A) Binding of FGF10 to HSPG is increased when compared with FGF7 in confluent  20-3 lung epithelial cells; however, binding to FGFR2 is similar for both FGFs (see  Materials and methods).	bind
54107	5	2617	5	10	NULL	0	NULL	statement 3	Process		is similar to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_258_1_185_s_123	12781692	(A) Binding of FGF10 to HSPG is increased when compared with FGF7 in confluent  20-3 lung epithelial cells; however, binding to FGFR2 is similar for both FGFs (see  Materials and methods).	bind
7151	1	2617	7	10	NULL	0	NULL	FGF10	GP		binds					 HSPG	GP				NULL	confluent 20-3 lung epithelial cells	NULL	NULL	NULL	NULL	gw70_devbiol_258_1_185_s_123	12781692	(A) Binding of FGF10 to HSPG is increased when compared with FGF7 in confluent  20-3 lung epithelial cells; however, binding to FGFR2 is similar for both FGFs (see  Materials and methods).	bind
7152	2	2617	7	10	NULL	0	NULL	FGF7	GP		binds					HSPG	GP				NULL	confluent 20-3 lung epithelial cells	NULL	NULL	NULL	NULL	gw70_devbiol_258_1_185_s_123	12781692	(A) Binding of FGF10 to HSPG is increased when compared with FGF7 in confluent  20-3 lung epithelial cells; however, binding to FGFR2 is similar for both FGFs (see  Materials and methods).	bind
7154	3	2617	7	10	NULL	0	NULL	FGF10	GP		binds to					FGFR2	GP				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_258_1_185_s_123	12781692	(A) Binding of FGF10 to HSPG is increased when compared with FGF7 in confluent  20-3 lung epithelial cells; however, binding to FGFR2 is similar for both FGFs (see  Materials and methods).	bind
7155	4	2617	7	10	NULL	0	NULL	FGF7	GP		binds to					FGFR2	GP				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_258_1_185_s_123	12781692	(A) Binding of FGF10 to HSPG is increased when compared with FGF7 in confluent  20-3 lung epithelial cells; however, binding to FGFR2 is similar for both FGFs (see  Materials and methods).	bind
54108	5	2617	7	10	NULL	0	NULL	statement 3	Process		is similar to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_258_1_185_s_123	12781692	(A) Binding of FGF10 to HSPG is increased when compared with FGF7 in confluent  20-3 lung epithelial cells; however, binding to FGFR2 is similar for both FGFs (see  Materials and methods).	bind
4819	1	2619	5	10	NULL	0	NULL	GAGA protein	GP		bind					iab-7	GP			PRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_4_1311_s_159	11158316	(A) Binding of GAGA protein to the  iab-7 PRE.	bind
7156	1	2619	7	10	NULL	0	NULL	GAGA protein	GP		binds					iab-7	GP			PRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_4_1311_s_159	11158316	(A) Binding of GAGA protein to the  iab-7 PRE.	bind
4820	1	2620	5	10	NULL	0	NULL	Rab9	GP	GST	bind					EEA1	GP				NULL	cytosol	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_77	16769818	(A) Binding of GST versions of Rab9, Rab5, Rab9/5, and Rab5/9 to Rab5 effectors EEA1  and rabaptin-5 from cytosol.	bind
4821	2	2620	5	10	NULL	0	NULL	Rab9	GP	GST	bind					rabaptin-5	GP				NULL	cytosol	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_77	16769818	(A) Binding of GST versions of Rab9, Rab5, Rab9/5, and Rab5/9 to Rab5 effectors EEA1  and rabaptin-5 from cytosol.	bind
4822	3	2620	5	10	NULL	0	NULL	Rab5	GP	GST	bind					EEA1	GP				NULL	cytosol	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_77	16769818	(A) Binding of GST versions of Rab9, Rab5, Rab9/5, and Rab5/9 to Rab5 effectors EEA1  and rabaptin-5 from cytosol.	bind
4823	4	2620	5	10	NULL	0	NULL	Rab5	GP	GST	bind					rabaptin-5	GP				NULL	cytosol	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_77	16769818	(A) Binding of GST versions of Rab9, Rab5, Rab9/5, and Rab5/9 to Rab5 effectors EEA1  and rabaptin-5 from cytosol.	bind
4824	5	2620	5	10	NULL	0	NULL	Rab9/5	GP	GST	bind					EEA1	GP				NULL	cytosol	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_77	16769818	(A) Binding of GST versions of Rab9, Rab5, Rab9/5, and Rab5/9 to Rab5 effectors EEA1  and rabaptin-5 from cytosol.	bind
4825	6	2620	5	10	NULL	0	NULL	Rab9/5	GP	GST 	bind					rabaptin-5	GP				NULL	cytosol	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_77	16769818	(A) Binding of GST versions of Rab9, Rab5, Rab9/5, and Rab5/9 to Rab5 effectors EEA1  and rabaptin-5 from cytosol.	bind
4826	7	2620	5	10	NULL	0	NULL	Rab5/9	GP	GST	bind					EEA1	GP				NULL	cytosol	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_77	16769818	(A) Binding of GST versions of Rab9, Rab5, Rab9/5, and Rab5/9 to Rab5 effectors EEA1  and rabaptin-5 from cytosol.	bind
4827	8	2620	5	10	NULL	0	NULL	Rab5/9	GP	GST	bind					rabaptin-5	GP				NULL	cytosol	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_77	16769818	(A) Binding of GST versions of Rab9, Rab5, Rab9/5, and Rab5/9 to Rab5 effectors EEA1  and rabaptin-5 from cytosol.	bind
46242	9	2620	5	10	NULL	0	NULL	EEA1	GP		is a type of					Rab5 effector	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_77	16769818	(A) Binding of GST versions of Rab9, Rab5, Rab9/5, and Rab5/9 to Rab5 effectors EEA1  and rabaptin-5 from cytosol.	bind
46243	10	2620	5	10	NULL	0	NULL	rabaptin-5	GP		is a type of					Rab5 effector	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_77	16769818	(A) Binding of GST versions of Rab9, Rab5, Rab9/5, and Rab5/9 to Rab5 effectors EEA1  and rabaptin-5 from cytosol.	bind
7157	1	2620	7	10	NULL	0	NULL	Rab9	GP	GST	binds					EEA1 	GP				NULL	cytosol	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_77	16769818	(A) Binding of GST versions of Rab9, Rab5, Rab9/5, and Rab5/9 to Rab5 effectors EEA1  and rabaptin-5 from cytosol.	bind
7158	2	2620	7	10	NULL	0	NULL	Rab9	GP	GST	binds					rabaptin-5	GP				NULL	cytosol	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_77	16769818	(A) Binding of GST versions of Rab9, Rab5, Rab9/5, and Rab5/9 to Rab5 effectors EEA1  and rabaptin-5 from cytosol.	bind
7159	3	2620	7	10	NULL	0	NULL	Rab5	GP	GST	binds					EEA1 	GP				NULL	cytosol	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_77	16769818	(A) Binding of GST versions of Rab9, Rab5, Rab9/5, and Rab5/9 to Rab5 effectors EEA1  and rabaptin-5 from cytosol.	bind
7160	4	2620	7	10	NULL	0	NULL	Rab5	GP	GST	binds					rabaptin-5	GP				NULL	cytosol	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_77	16769818	(A) Binding of GST versions of Rab9, Rab5, Rab9/5, and Rab5/9 to Rab5 effectors EEA1  and rabaptin-5 from cytosol.	bind
7161	5	2620	7	10	NULL	0	NULL	Rab9/5	GP	GST	binds					EEA1 	GP				NULL	cytosol	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_77	16769818	(A) Binding of GST versions of Rab9, Rab5, Rab9/5, and Rab5/9 to Rab5 effectors EEA1  and rabaptin-5 from cytosol.	bind
7162	6	2620	7	10	NULL	0	NULL	Rab9/5	GP	GST	binds					rabaptin-5	GP				NULL	cytosol	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_77	16769818	(A) Binding of GST versions of Rab9, Rab5, Rab9/5, and Rab5/9 to Rab5 effectors EEA1  and rabaptin-5 from cytosol.	bind
7163	7	2620	7	10	NULL	0	NULL	Rab5/9	GP	GST	binds					EEA1 	GP				NULL	cytosol	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_77	16769818	(A) Binding of GST versions of Rab9, Rab5, Rab9/5, and Rab5/9 to Rab5 effectors EEA1  and rabaptin-5 from cytosol.	bind
7164	8	2620	7	10	NULL	0	NULL	Rab5/9	GP	GST	binds					rabaptin-5	GP				NULL	cytosol	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_77	16769818	(A) Binding of GST versions of Rab9, Rab5, Rab9/5, and Rab5/9 to Rab5 effectors EEA1  and rabaptin-5 from cytosol.	bind
46244	9	2620	7	10	NULL	0	NULL	EEA1	GP		is a type of					Rab5 effector	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_77	16769818	(A) Binding of GST versions of Rab9, Rab5, Rab9/5, and Rab5/9 to Rab5 effectors EEA1  and rabaptin-5 from cytosol.	bind
46245	10	2620	7	10	NULL	0	NULL	rabaptin-5	GP		is a type of					Rab5 effector	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_77	16769818	(A) Binding of GST versions of Rab9, Rab5, Rab9/5, and Rab5/9 to Rab5 effectors EEA1  and rabaptin-5 from cytosol.	bind
4828	1	2621	5	10	NULL	0	NULL	GTP	Chemical		bind					Rac	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_293_5_1571_s_121	12054696	(A) Binding of GST-PAK2-RBD to the GTP-bound form of Rac.	bind
46246	2	2621	5	10	NULL	0	NULL	GST-PAK2	GP		bind			RBD		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_293_5_1571_s_121	12054696	(A) Binding of GST-PAK2-RBD to the GTP-bound form of Rac.	bind
7167	1	2621	7	10	NULL	0	NULL	GTP	Chemical		bind					Rac	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_293_5_1571_s_121	12054696	(A) Binding of GST-PAK2-RBD to the GTP-bound form of Rac.	bind
46248	2	2621	7	10	NULL	0	NULL	GST-PAK2	GP		bind			RBD		statement1	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_293_5_1571_s_121	12054696	(A) Binding of GST-PAK2-RBD to the GTP-bound form of Rac.	bind
4829	1	2622	5	10	NULL	0	NULL	GST-s-synaphin	GP		bind					r-syntaxin	GP	recombinant			NULL		NULL	NULL	NULL	NULL	gw60_cell_104_3_421_s_54	11239399	(A) Binding of GST-s-synaphin to recombinant r-syntaxin in the presence or absence of r-SNAP-25 (1 muM) and/or r-synaptobrevin 2 (2 muM), or both.	bind
7168	1	2622	7	10	NULL	0	NULL	GST-s-synaphin	GP		binds					r-syntaxin	GP	recombinant			NULL		NULL	NULL	NULL	NULL	gw60_cell_104_3_421_s_54	11239399	(A) Binding of GST-s-synaphin to recombinant r-syntaxin in the presence or absence of r-SNAP-25 (1 muM) and/or r-synaptobrevin 2 (2 muM), or both.	bind
4839	1	2623	5	10	NULL	0	NULL	hMutS	GP		bind					substrates	GP	containing two-nucleotide loops			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_9_1181_s_51	8805365	(a) Binding of hMutS  and hMutS  to substrates containing two-nucleotide loops.	bind
7170	1	2623	7	10	NULL	0	NULL	hMutS	GP		binds to					substrates	GP	containing two-nucleotide loops			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_9_1181_s_51	8805365	(a) Binding of hMutS  and hMutS  to substrates containing two-nucleotide loops.	bind
4841	1	2624	5	10	NULL	0	NULL	IL-15 IgG 2b	GP		bind					PMN	Cell				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_6_2640_s_109	9596728	(A) Binding of IL-15 IgG 2b fusion protein to PMN.	bind
46254	2	2624	5	10	NULL	0	NULL	IL-15 IgG 2b	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_6_2640_s_109	9596728	(A) Binding of IL-15 IgG 2b fusion protein to PMN.	bind
7171	1	2624	7	10	NULL	0	NULL	IL-15 IgG 2b	GP		binds					PMN	Cell				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_6_2640_s_109	9596728	(A) Binding of IL-15 IgG 2b fusion protein to PMN.	bind
46255	2	2624	7	10	NULL	0	NULL	IL-15 IgG 2b	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_6_2640_s_109	9596728	(A) Binding of IL-15 IgG 2b fusion protein to PMN.	bind
4842	1	2626	5	NULL	NULL	0	NULL		NULL	isolated	bind	NULL		PDZ domains		PIP2 micelles	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_9_6_1215_s_133	12086619	(A) Binding of isolated PDZ domains to PIP2 micelles.	bind
7172	1	2626	7	NULL	NULL	0	NULL		NULL	isolated	binds	NULL		PDZ domains		PIP2 micelles	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_9_6_1215_s_133	12086619	(A) Binding of isolated PDZ domains to PIP2 micelles.	bind
4843	1	2627	5	10	NULL	0	NULL	JSAP1	GP		bind					MAPKKKs	GP	mammalian			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_11_7539_s_285	10523642	(A) Binding of JSAP1 to mammalian MAPKKKs.	bind
7173	1	2627	7	10	NULL	0	NULL	JSAP1	GP		binds to					MAPKKK	GP	mammalian			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_11_7539_s_285	10523642	(A) Binding of JSAP1 to mammalian MAPKKKs.	bind
4846	1	2630	5	10	NULL	0	NULL	lens cell extracts	Cell		bind					zeta ZPE	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2067_s_150	9528779	(a) Binding of lens cell extracts and recombinant Pax6 proteins to the zeta ZPE.	bind
4847	2	2630	5	10	NULL	0	NULL	Pax6 protein	GP	recombinant	bind					zeta ZPE	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2067_s_150	9528779	(a) Binding of lens cell extracts and recombinant Pax6 proteins to the zeta ZPE.	bind
7186	1	2630	7	10	NULL	0	NULL	lens cell extracts	Cell		binds					 zeta ZPE	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2067_s_150	9528779	(a) Binding of lens cell extracts and recombinant Pax6 proteins to the zeta ZPE.	bind
7187	2	2630	7	10	NULL	0	NULL	Pax6	GP	recombinant	binds					zeta ZPE	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2067_s_150	9528779	(a) Binding of lens cell extracts and recombinant Pax6 proteins to the zeta ZPE.	bind
4848	1	2631	5	10	NULL	0	NULL	Mbt	GP		bind					Rho-type GTPases	GP				NULL		NULL	NULL	NULL	NULL	gw60_development_130_3_427_s_171	12490550	(A) Binding of Mbt to Rho-type GTPases.	bind
7188	1	2631	7	10	NULL	0	NULL	Mbt	GP		binds					Rho-type GTPases	GP				NULL		NULL	NULL	NULL	NULL	gw60_development_130_3_427_s_171	12490550	(A) Binding of Mbt to Rho-type GTPases.	bind
4849	1	2632	5	10	NULL	0	NULL	LGN	GP	mouse	bind					heterotrimeric G-proteins	GP	Galpha subunits of			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_8_3144_s_251	12925752	(A) Binding of mouse LGN to Galpha subunits of  heterotrimeric G-proteins.	bind
7189	1	2632	7	10	NULL	0	NULL	LGN	GP	mouse	binds					heterotrimeric G-proteins	GP	Galpha subunits of 			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_8_3144_s_251	12925752	(A) Binding of mouse LGN to Galpha subunits of  heterotrimeric G-proteins.	bind
4850	1	2633	5	10	NULL	0	NULL	myosin-VIIa	GP		bind			tail		GST	Chemical	purified			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_163_3_559_s_122	14610058	(A) Binding of myosin-VIIa tail (left) or myosin-Va (middle) to purified GST or GST  - MyRIP constructs immobilized on glutathione - Sepharose beads.	bind
4851	2	2633	5	10	NULL	0	NULL	myosin-Va	GP		bind					GST	Chemical	purified			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_163_3_559_s_122	14610058	(A) Binding of myosin-VIIa tail (left) or myosin-Va (middle) to purified GST or GST  - MyRIP constructs immobilized on glutathione - Sepharose beads.	bind
4852	3	2633	5	10	NULL	0	NULL	myosin-VIIa	GP		bind			tail		GST - MyRIP	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_163_3_559_s_122	14610058	(A) Binding of myosin-VIIa tail (left) or myosin-Va (middle) to purified GST or GST  - MyRIP constructs immobilized on glutathione - Sepharose beads.	bind
4853	4	2633	5	10	NULL	0	NULL	myosin-Va	GP		bind					GST - MyRIP	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_163_3_559_s_122	14610058	(A) Binding of myosin-VIIa tail (left) or myosin-Va (middle) to purified GST or GST  - MyRIP constructs immobilized on glutathione - Sepharose beads.	bind
7281	1	2633	7	10	NULL	0	NULL	myosin-VIIa	GP		binds			tail		GST	Chemical	purified			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_163_3_559_s_122	14610058	(A) Binding of myosin-VIIa tail (left) or myosin-Va (middle) to purified GST or GST  - MyRIP constructs immobilized on glutathione - Sepharose beads.	bind
7282	2	2633	7	10	NULL	0	NULL	myosin-VIIa	GP		binds			tail		GST - MyRIP	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_163_3_559_s_122	14610058	(A) Binding of myosin-VIIa tail (left) or myosin-Va (middle) to purified GST or GST  - MyRIP constructs immobilized on glutathione - Sepharose beads.	bind
7283	3	2633	7	10	NULL	0	NULL	myosin-Va	GP		binds					GST	Chemical	purified			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_163_3_559_s_122	14610058	(A) Binding of myosin-VIIa tail (left) or myosin-Va (middle) to purified GST or GST  - MyRIP constructs immobilized on glutathione - Sepharose beads.	bind
7284	4	2633	7	10	NULL	0	NULL	myosin-Va	GP		binds					GST - MyRIP	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_163_3_559_s_122	14610058	(A) Binding of myosin-VIIa tail (left) or myosin-Va (middle) to purified GST or GST  - MyRIP constructs immobilized on glutathione - Sepharose beads.	bind
4854	1	2634	5	10	NULL	0	NULL	n-sec1	GP		bind					syntaxin 1a	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_16_6_1229_s_88	8663999	(A) Binding of n-sec1 to syntaxin 1a in the absence of NO.	bind
4855	2	2634	5	10	NULL	0	NULL	statement 1	GP		in the absence of					NO	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neuron_16_6_1229_s_88	8663999	(A) Binding of n-sec1 to syntaxin 1a in the absence of NO.	bind
7285	1	2634	7	10	NULL	0	NULL	 n-sec1	GP		binds to					syntaxin 1a	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_16_6_1229_s_88	8663999	(A) Binding of n-sec1 to syntaxin 1a in the absence of NO.	bind
7286	2	2634	7	10	NULL	0	NULL	statement 1	Process		occurs in the absence of					NO	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neuron_16_6_1229_s_88	8663999	(A) Binding of n-sec1 to syntaxin 1a in the absence of NO.	bind
5565	1	2635	5	10	NULL	0	NULL	NusA	GP		bind					N. NusA	GP	deletion mutants of	amino-terminal		NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_265_s_133	9659923	(A) Binding of NusA and RNAP to amino-terminal deletion mutants of N. NusA (lane 2) or RNAP (lane 10) was loaded onto 0.5 mg/ml GST, GST-N73-107, GST-N58-107, GST-N48-107, GST-N34-107, GST-N23-107, and GST-N columns (as indicated).	bind
5567	2	2635	5	10	NULL	0	NULL	NusA	GP		bind					RNAP	GP	deletion mutants of	amino-terminal		NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_265_s_133	9659923	(A) Binding of NusA and RNAP to amino-terminal deletion mutants of N. NusA (lane 2) or RNAP (lane 10) was loaded onto 0.5 mg/ml GST, GST-N73-107, GST-N58-107, GST-N48-107, GST-N34-107, GST-N23-107, and GST-N columns (as indicated).	bind
5568	3	2635	5	10	NULL	0	NULL	RNAP	GP		bind					N. NusA	GP	deletion mutants of	amino-terminal 		NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_265_s_133	9659923	(A) Binding of NusA and RNAP to amino-terminal deletion mutants of N. NusA (lane 2) or RNAP (lane 10) was loaded onto 0.5 mg/ml GST, GST-N73-107, GST-N58-107, GST-N48-107, GST-N34-107, GST-N23-107, and GST-N columns (as indicated).	bind
5570	4	2635	5	10	NULL	0	NULL	RNAP	GP		bind					RNAP	GP	deletion mutants of	amino-terminal 		NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_265_s_133	9659923	(A) Binding of NusA and RNAP to amino-terminal deletion mutants of N. NusA (lane 2) or RNAP (lane 10) was loaded onto 0.5 mg/ml GST, GST-N73-107, GST-N58-107, GST-N48-107, GST-N34-107, GST-N23-107, and GST-N columns (as indicated).	bind
7287	1	2635	7	10	NULL	0	NULL	NusA	GP		binds					N. NusA	GP	deletion mutants of	amino-terminal 		NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_265_s_133	9659923	(A) Binding of NusA and RNAP to amino-terminal deletion mutants of N. NusA (lane 2) or RNAP (lane 10) was loaded onto 0.5 mg/ml GST, GST-N73-107, GST-N58-107, GST-N48-107, GST-N34-107, GST-N23-107, and GST-N columns (as indicated).	bind
7288	2	2635	7	10	NULL	0	NULL	RNAP	GP		binds					N. NusA	GP	deletion mutants of	amino-terminal 		NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_265_s_133	9659923	(A) Binding of NusA and RNAP to amino-terminal deletion mutants of N. NusA (lane 2) or RNAP (lane 10) was loaded onto 0.5 mg/ml GST, GST-N73-107, GST-N58-107, GST-N48-107, GST-N34-107, GST-N23-107, and GST-N columns (as indicated).	bind
7289	3	2635	7	10	NULL	0	NULL	NusA	GP		binds					RNAP	GP	deletion mutants of	amino-terminal 		NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_265_s_133	9659923	(A) Binding of NusA and RNAP to amino-terminal deletion mutants of N. NusA (lane 2) or RNAP (lane 10) was loaded onto 0.5 mg/ml GST, GST-N73-107, GST-N58-107, GST-N48-107, GST-N34-107, GST-N23-107, and GST-N columns (as indicated).	bind
7290	4	2635	7	10	NULL	0	NULL	RNAP	GP		binds					RNAP	GP	deletion mutants of	amino-terminal		NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_265_s_133	9659923	(A) Binding of NusA and RNAP to amino-terminal deletion mutants of N. NusA (lane 2) or RNAP (lane 10) was loaded onto 0.5 mg/ml GST, GST-N73-107, GST-N58-107, GST-N48-107, GST-N34-107, GST-N23-107, and GST-N columns (as indicated).	bind
5269	1	2636	5	10	NULL	0	NULL	p34 cdc2	GP		bind					CksHs2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_3659_s_214	9632748	(A) Binding of p34 cdc2 and cyclin B to CksHs2-Sepharose beads.	bind
5270	2	2636	5	10	NULL	0	NULL	cyclin B	GP		bind					CksHs2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_3659_s_214	9632748	(A) Binding of p34 cdc2 and cyclin B to CksHs2-Sepharose beads.	bind
7291	1	2636	7	10	NULL	0	NULL	p34 cdc2	GP		binds					CksHs2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_3659_s_214	9632748	(A) Binding of p34 cdc2 and cyclin B to CksHs2-Sepharose beads.	bind
7292	2	2636	7	10	NULL	0	NULL	cyclin B	GP		binds					CksHs2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_3659_s_214	9632748	(A) Binding of p34 cdc2 and cyclin B to CksHs2-Sepharose beads.	bind
5271	1	2637	5	10	NULL	0	NULL	pb2-DHFR	GP		bind					mitochondria	CellComponent	mutant			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1509_1_86_s_128	11118520	(A) Binding of pb2-DHFR with mutant mitochondria (MITO) and mitoplasts (MTP) in the absence of the inner membrane potential (-   ).	bind
5272	2	2637	5	10	NULL	0	NULL	statement 1	Process		in the absence of					inner membrane potential					NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1509_1_86_s_128	11118520	(A) Binding of pb2-DHFR with mutant mitochondria (MITO) and mitoplasts (MTP) in the absence of the inner membrane potential (-   ).	bind
5273	3	2637	5	10	NULL	0	NULL	pb2-DHFR	GP		bind					mitoplasts	CellComponent	mutant			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1509_1_86_s_128	11118520	(A) Binding of pb2-DHFR with mutant mitochondria (MITO) and mitoplasts (MTP) in the absence of the inner membrane potential (-   ).	bind
5274	4	2637	5	10	NULL	0	NULL	statement 3	Process		in the absence of					inner membrane potential					NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1509_1_86_s_128	11118520	(A) Binding of pb2-DHFR with mutant mitochondria (MITO) and mitoplasts (MTP) in the absence of the inner membrane potential (-   ).	bind
54130	5	2637	5	10	NULL	0	NULL	MITO	CellComponent		is					mitochondria	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1509_1_86_s_128	11118520	(A) Binding of pb2-DHFR with mutant mitochondria (MITO) and mitoplasts (MTP) in the absence of the inner membrane potential (-   ).	bind
54131	6	2637	5	10	NULL	0	NULL	MTP	CellComponent		is					mitoplast	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1509_1_86_s_128	11118520	(A) Binding of pb2-DHFR with mutant mitochondria (MITO) and mitoplasts (MTP) in the absence of the inner membrane potential (-   ).	bind
7293	1	2637	7	10	NULL	0	NULL	pb2-DHFR	GP		binds					mitochondria	CellComponent	mutant			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1509_1_86_s_128	11118520	(A) Binding of pb2-DHFR with mutant mitochondria (MITO) and mitoplasts (MTP) in the absence of the inner membrane potential (-   ).	bind
7294	2	2637	7	10	NULL	0	NULL	pb2-DHFR	GP		binds					mitoplasts	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1509_1_86_s_128	11118520	(A) Binding of pb2-DHFR with mutant mitochondria (MITO) and mitoplasts (MTP) in the absence of the inner membrane potential (-   ).	bind
7295	3	2637	7	10	NULL	0	NULL	MITO	CellComponent		is					mitochondria	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1509_1_86_s_128	11118520	(A) Binding of pb2-DHFR with mutant mitochondria (MITO) and mitoplasts (MTP) in the absence of the inner membrane potential (-   ).	bind
7296	4	2637	7	10	NULL	0	NULL	MTP	CellComponent		is					mitoplasts	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1509_1_86_s_128	11118520	(A) Binding of pb2-DHFR with mutant mitochondria (MITO) and mitoplasts (MTP) in the absence of the inner membrane potential (-   ).	bind
54132	5	2637	7	10	NULL	0	NULL	statement 1	Process		occurs in the absence of					inner membrane potential					NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1509_1_86_s_128	11118520	(A) Binding of pb2-DHFR with mutant mitochondria (MITO) and mitoplasts (MTP) in the absence of the inner membrane potential (-   ).	bind
54133	6	2637	7	10	NULL	0	NULL	statement 2	Process		occurs in the absence of					inner membrane potential					NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1509_1_86_s_128	11118520	(A) Binding of pb2-DHFR with mutant mitochondria (MITO) and mitoplasts (MTP) in the absence of the inner membrane potential (-   ).	bind
5275	1	2638	5	10	NULL	0	NULL	PP1	GP		bind					AKAP149	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_150_6_1251_s_163	10995432	(A) Binding of PP1 to AKAP149.	bind
7297	1	2638	7	10	NULL	0	NULL	PP1	GP		binds					AKAP149	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_150_6_1251_s_163	10995432	(A) Binding of PP1 to AKAP149.	bind
5276	1	2639	5	10	NULL	0	NULL	pRb	GP		bind					GST-CBFA1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_2_303_s_205	11545733	(A) Binding of pRb and tumor-derived mutants expressed in Cos cells to GST-CBFA1 or GST.	bind
5277	2	2639	5	10	NULL	0	NULL	pRb	GP		bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_2_303_s_205	11545733	(A) Binding of pRb and tumor-derived mutants expressed in Cos cells to GST-CBFA1 or GST.	bind
5278	3	2639	5	10	NULL	0	NULL	tumor-derived mutants	GP	expressed in Cos cells	bind					GST-CBFA1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_2_303_s_205	11545733	(A) Binding of pRb and tumor-derived mutants expressed in Cos cells to GST-CBFA1 or GST.	bind
5279	4	2639	5	10	NULL	0	NULL	tumor-derived mutants	GP	expressed in Cos cells	bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_2_303_s_205	11545733	(A) Binding of pRb and tumor-derived mutants expressed in Cos cells to GST-CBFA1 or GST.	bind
7298	1	2639	7	10	NULL	0	NULL	pRb	GP		binds					GST-CBFA1 	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_2_303_s_205	11545733	(A) Binding of pRb and tumor-derived mutants expressed in Cos cells to GST-CBFA1 or GST.	bind
7299	2	2639	7	10	NULL	0	NULL	pRb	GP		binds					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_2_303_s_205	11545733	(A) Binding of pRb and tumor-derived mutants expressed in Cos cells to GST-CBFA1 or GST.	bind
7300	3	2639	7	10	NULL	0	NULL	tumor-derived mutants	GP	expressed in cos cells	binds to					GST-CBFA1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_2_303_s_205	11545733	(A) Binding of pRb and tumor-derived mutants expressed in Cos cells to GST-CBFA1 or GST.	bind
7301	4	2639	7	10	NULL	0	NULL	tumor-derived mutants	GP	expressed in cos cells	binds					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_2_303_s_205	11545733	(A) Binding of pRb and tumor-derived mutants expressed in Cos cells to GST-CBFA1 or GST.	bind
5280	2	2640	5	10	NULL	0	NULL	olfactory epithelial nuclear proteins	GP	rat	bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_72_1_65_s_104	10521600	(A) Binding of rat olfactory epithelial nuclear proteins with putative NFI-binding sites from genes expressed abundantly within the olfactory epithelium.	bind
5281	1	2640	5	10	NULL	0	NULL	genes	GP		is expressed		abundantly		NFI-binding sites	olfactory epithelium	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_72_1_65_s_104	10521600	(A) Binding of rat olfactory epithelial nuclear proteins with putative NFI-binding sites from genes expressed abundantly within the olfactory epithelium.	bind
7302	1	2640	7	10	NULL	0	NULL	olfactory epithelial nuclear proteins	GP	rat	binds							putative		NFI-binding sites	NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_72_1_65_s_104	10521600	(A) Binding of rat olfactory epithelial nuclear proteins with putative NFI-binding sites from genes expressed abundantly within the olfactory epithelium.	bind
7303	2	2640	7	10	NULL	0	NULL	genes	GP		is expressed in		abundantly		NFI-binding sites	olfactory epithelium	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_72_1_65_s_104	10521600	(A) Binding of rat olfactory epithelial nuclear proteins with putative NFI-binding sites from genes expressed abundantly within the olfactory epithelium.	bind
5282	1	2641	5	10	NULL	0	NULL	RIN1	GP		bind					GST-RAS	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_3_916_s_136	11784866	(A) Binding of RIN1 to GST-RAS.	bind
7304	1	2641	7	10	NULL	0	NULL	RIN1	GP		binds					GST-RAS	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_3_916_s_136	11784866	(A) Binding of RIN1 to GST-RAS.	bind
5283	1	2642	5	10	NULL	0	NULL	RNCs	GP		bind					TX-PK-RM	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_150_1_53_s_182	10893256	(A) Binding of RNCs to TX-PK-RM was assayed by adjusting samples to 2.1 M sucrose and applying them as the bottom layer of a three-step discontinuous sucrose gradient (see Materials and Methods).	bind
7305	1	2642	7	10	NULL	0	NULL	RNCs	GP		binds to					TX-PK-RM	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_150_1_53_s_182	10893256	(A) Binding of RNCs to TX-PK-RM was assayed by adjusting samples to 2.1 M sucrose and applying them as the bottom layer of a three-step discontinuous sucrose gradient (see Materials and Methods).	bind
5284	1	2643	5	10	NULL	0	NULL	syncollin	GP		bind					GST-syntaxin fragments	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_90_2_325_s_68	9244306	(A) Binding of syncollin to various  GST-syntaxin fragments.	bind
7306	1	2643	7	10	NULL	0	NULL	syncollin	GP		binds to					GST-syntaxin fragments	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_90_2_325_s_68	9244306	(A) Binding of syncollin to various  GST-syntaxin fragments.	bind
5285	1	2644	5	10	NULL	0	NULL	syntaxin-1a	GP		bind					tomosyn	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_20_5_905_s_136	9620695	(A) Binding of syntaxin-1a to tomosyn.	bind
7307	1	2644	7	10	NULL	0	NULL	syntaxin-1a	GP		binds					tomosyn	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_20_5_905_s_136	9620695	(A) Binding of syntaxin-1a to tomosyn.	bind
5286	1	2645	5	10	NULL	0	NULL	TFs	GP		bind					c-fos	GP	human		SRE	NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1574_1_100_s_51	11955618	(A) Binding of TFs to the human c-fos SRE.	bind
7308	1	2645	7	10	NULL	0	NULL	TF	GP		binds					c-fos	GP	human		SRE	NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1574_1_100_s_51	11955618	(A) Binding of TFs to the human c-fos SRE.	bind
5287	1	2646	5	10	NULL	0	NULL	eEF1 complex	GP		bind					G-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1527_3_130_s_236	11479029	(A) Binding of the eEF1   complex to G-actin.	bind
7309	1	2646	7	10	NULL	0	NULL	eEF1 complex	GP		binds to					G-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1527_3_130_s_236	11479029	(A) Binding of the eEF1   complex to G-actin.	bind
7176	1	2648	5	10	NULL	0	NULL				bind			Skn domain		DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_3039_s_105	10082571	(A) Binding of the Skn domain and the delta1-9 Skn domain mutant ( 2) to DNA, assayed by EMSA at room temperature (RT).	bind
54137	2	2648	5	10	NULL	0	NULL			mutant	bind			delta1-9 Skn domain		DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_3039_s_105	10082571	(A) Binding of the Skn domain and the delta1-9 Skn domain mutant ( 2) to DNA, assayed by EMSA at room temperature (RT).	bind
7326	1	2648	7	10	NULL	0	NULL				binds			Skn domain		DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_3039_s_105	10082571	(A) Binding of the Skn domain and the delta1-9 Skn domain mutant ( 2) to DNA, assayed by EMSA at room temperature (RT).	bind
7327	2	2648	7	10	NULL	0	NULL			mutant	binds			delta1-9 Skn domain		DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_3039_s_105	10082571	(A) Binding of the Skn domain and the delta1-9 Skn domain mutant ( 2) to DNA, assayed by EMSA at room temperature (RT).	bind
5288	1	2649	5	10	NULL	0	NULL	thyroglobulin	GP		bind					SpeB extracts	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_71_2_784_s_141	12540558	(A) Binding of thyroglobulin to SpeB extracts of the  rgg mutant strain NZ131 rgg.	bind
46257	2	2649	5	10	NULL	0	NULL	SpeB extracts	GP		are derived from					NZ131 rgg strain	Organism	mutant			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_71_2_784_s_141	12540558	(A) Binding of thyroglobulin to SpeB extracts of the  rgg mutant strain NZ131 rgg.	bind
7328	1	2649	7	10	NULL	0	NULL	thyroglobulin	GP		binds to					SpeB extracts	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_71_2_784_s_141	12540558	(A) Binding of thyroglobulin to SpeB extracts of the  rgg mutant strain NZ131 rgg.	bind
7329	2	2649	7	10	NULL	0	NULL	SpeB extracts	GP		is derived from	Organism				NZ131 rgg strain	Organism	mutant			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_71_2_784_s_141	12540558	(A) Binding of thyroglobulin to SpeB extracts of the  rgg mutant strain NZ131 rgg.	bind
5289	1	2650	5	10	NULL	0	NULL	Vav-3	GP		bind			delta1-144		Rho family proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_11_7870_s_267	10523675	(A) Binding of Vav-3 (delta1-144) to Rho family proteins.	bind
7330	1	2650	7	10	NULL	0	NULL	Vav-3	GP		binds to			delta1-144		Rho family proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_11_7870_s_267	10523675	(A) Binding of Vav-3 (delta1-144) to Rho family proteins.	bind
5290	1	2651	5	10	NULL	0	NULL	VEGF-E	GP		bind					VEGFR - IgG	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_161_6_1163_s_247	12810700	(a) Binding of VEGF-E to VEGFR - IgG fusion proteins.	bind
46260	2	2651	5	10	NULL	0	NULL	VEGFR- IgG	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_161_6_1163_s_247	12810700	(a) Binding of VEGF-E to VEGFR - IgG fusion proteins.	bind
7332	1	2651	7	10	NULL	0	NULL	VEGF-E	GP		binds to					VEGFR - IgG 	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_161_6_1163_s_247	12810700	(a) Binding of VEGF-E to VEGFR - IgG fusion proteins.	bind
46261	2	2651	7	10	NULL	0	NULL	VEGFR- IgG	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_161_6_1163_s_247	12810700	(a) Binding of VEGF-E to VEGFR - IgG fusion proteins.	bind
5291	1	2652	5	10	NULL	0	NULL	vitronectin	GP		bind					UspA1	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_9_4374_s_274	9712790	(A) Binding of vitronectin to UspA1 and UspA2.	bind
5292	2	2652	5	10	NULL	0	NULL	vitronectin	GP		bind					UspA2	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_9_4374_s_274	9712790	(A) Binding of vitronectin to UspA1 and UspA2.	bind
7333	1	2652	7	10	NULL	0	NULL	vitronectin	GP		binds to					UspA1	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_9_4374_s_274	9712790	(A) Binding of vitronectin to UspA1 and UspA2.	bind
7334	2	2652	7	10	NULL	0	NULL	vitronectin	GP		binds to					UspA2	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_9_4374_s_274	9712790	(A) Binding of vitronectin to UspA1 and UspA2.	bind
5293	1	2653	5	10	NULL	0	NULL	HGFSF	GP	wt	bind					Met-Fc	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_3_125_s_128	9443912	(a) Binding of wt-HGFSF and HP1 to Met-Fc.	bind
5294	2	2653	5	10	NULL	0	NULL	HP1	GP		bind					Met-Fc	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_3_125_s_128	9443912	(a) Binding of wt-HGFSF and HP1 to Met-Fc.	bind
7335	1	2653	7	10	NULL	0	NULL	HGFSF	GP	wt	binds to					Met-Fc	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_3_125_s_128	9443912	(a) Binding of wt-HGFSF and HP1 to Met-Fc.	bind
7336	2	2653	7	10	NULL	0	NULL	HP1	GP		binds to					Met-Fc	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_3_125_s_128	9443912	(a) Binding of wt-HGFSF and HP1 to Met-Fc.	bind
5295	1	2654	5	10	NULL	0	NULL	tpm3	GP	Wt	bind					F actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_2_300_s_99	12163017	(A) Binding of Wt-tpm3 to F actin and troponin.	bind
5296	2	2654	5	10	NULL	0	NULL	tpm3	GP	Wt	bind					troponin	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_2_300_s_99	12163017	(A) Binding of Wt-tpm3 to F actin and troponin.	bind
7337	1	2654	7	10	NULL	0	NULL	tpm3	GP	Wt	binds					F actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_2_300_s_99	12163017	(A) Binding of Wt-tpm3 to F actin and troponin.	bind
7338	2	2654	7	10	NULL	0	NULL	tpm3	GP	Wt	binds					troponin	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_2_300_s_99	12163017	(A) Binding of Wt-tpm3 to F actin and troponin.	bind
5297	1	2655	5	10	NULL	0	NULL	XIP-I	GP		bind					polysaccharides	Chemical	water-insoluble			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_136_s_195	12922177	(A) Binding of XIP-I or BASI to water-insoluble polysaccharides was measured as described in  Materials and methods.	bind
5298	2	2655	5	10	NULL	0	NULL	BASI	GP		bind					polysaccharides	Chemical	water-insoluble			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_136_s_195	12922177	(A) Binding of XIP-I or BASI to water-insoluble polysaccharides was measured as described in  Materials and methods.	bind
7339	1	2655	7	10	NULL	0	NULL	XIP-I	GP		binds					 polysaccharides	Chemical	water-insoluble			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_136_s_195	12922177	(A) Binding of XIP-I or BASI to water-insoluble polysaccharides was measured as described in  Materials and methods.	bind
7340	2	2655	7	10	NULL	0	NULL	BASI	GP		binds					polysaccharides	Chemical	water-insoluble			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_136_s_195	12922177	(A) Binding of XIP-I or BASI to water-insoluble polysaccharides was measured as described in  Materials and methods.	bind
5299	1	2656	5	10	NULL	0	NULL	XPC	GP		bind					nucleosomal DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_24_9173_s_167	11094069	(A) Binding of XPC to nucleosomal DNA.	bind
7341	1	2656	7	10	NULL	0	NULL	XPC	GP		binds to					nucleosomal DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_24_9173_s_167	11094069	(A) Binding of XPC to nucleosomal DNA.	bind
5300	1	2657	5	10	NULL	0	NULL	yeast cells	Cell		bind					BSA	Chemical	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_1_140_s_75	9423850	(A) Binding of yeast cells to BSA (BSA), effects of preincubation with BSA on binding of yeast cells to immobilized BSA (BSA/BSA) and following washout of free BSA [BSA(wash)/BSA], and effects of preincubation with gelatin on the binding of yeast cells to immobilized BSA (PreGel-BSA).	bind
7342	1	2657	7	10	NULL	0	NULL	yeast cells	Cell		binds					BSA	Chemical	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_1_140_s_75	9423850	(A) Binding of yeast cells to BSA (BSA), effects of preincubation with BSA on binding of yeast cells to immobilized BSA (BSA/BSA) and following washout of free BSA [BSA(wash)/BSA], and effects of preincubation with gelatin on the binding of yeast cells to immobilized BSA (PreGel-BSA).	bind
5301	1	2658	5	10	NULL	0	NULL	YopN	GP		bind					TyeA	GP				NULL	E.coli	NULL	NULL	NULL	NULL	gw60_embo_17_7_1907_s_166	9524114	(A) Binding of YopN to TyeA in  E.coli.	bind
7345	1	2658	7	10	NULL	0	NULL	YopN	GP		binds					TyeA	GP				NULL	E.coli	NULL	NULL	NULL	NULL	gw60_embo_17_7_1907_s_166	9524114	(A) Binding of YopN to TyeA in  E.coli.	bind
5302	1	2659	5	10	NULL	0	NULL	[3]SSO	Chemical		bind					DRMs	CellComponent				NULL	live cells	NULL	NULL	NULL	NULL	gw70_molbiolcell_16_1_24_s_147	15496455	(A) Binding of [3]SSO to DRMs of live cells.	bind
7346	1	2659	7	10	NULL	0	NULL	[3]SSO	Chemical		binds					DRMs	CellComponent				NULL	live cells	NULL	NULL	NULL	NULL	gw70_molbiolcell_16_1_24_s_147	15496455	(A) Binding of [3]SSO to DRMs of live cells.	bind
5303	1	2660	5	10	NULL	0	NULL	NAC	GP		bind					apoE	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_44_1_105_s_63	9030704	(A) Binding of []NAC to apoE in VLDL.	bind
5304	2	2660	5	10	NULL	0	NULL	statement 1	Process		occurs in					VLDL	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_44_1_105_s_63	9030704	(A) Binding of []NAC to apoE in VLDL.	bind
7347	1	2660	7	10	NULL	0	NULL	NAC	GP		binds					apoE	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_44_1_105_s_63	9030704	(A) Binding of []NAC to apoE in VLDL.	bind
8074	2	2660	7	10	NULL	0	NULL	statement 1	Process		occurs in					VLDL	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_44_1_105_s_63	9030704	(A) Binding of []NAC to apoE in VLDL.	bind
5870	1	2661	5	10	NULL	0	NULL	4F	GP		bind					cap analogue	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1678_2_67_s_1026	15157733	(A) binding protein  enhances the binding affinity of eukaryotic initiation factor 4F and (iso)4F for  cap analogues.	bind
5871	2	2661	5	10	NULL	0	NULL	(iso)4F	GP		bind					cap analogue	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1678_2_67_s_1026	15157733	(A) binding protein  enhances the binding affinity of eukaryotic initiation factor 4F and (iso)4F for  cap analogues.	bind
8179	3	2661	5	10	NULL	0	NULL	4F	GP		is a type of					eukaryotic initiation factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1678_2_67_s_1026	15157733	(A) binding protein  enhances the binding affinity of eukaryotic initiation factor 4F and (iso)4F for  cap analogues.	bind
8180	4	2661	5	10	NULL	0	NULL	(iso)4F	GP		is a type of					eukaryotic initiation factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1678_2_67_s_1026	15157733	(A) binding protein  enhances the binding affinity of eukaryotic initiation factor 4F and (iso)4F for  cap analogues.	bind
7348	1	2661	7	10	NULL	0	NULL	4F	GP		binds					cap analogues	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1678_2_67_s_1026	15157733	(A) binding protein  enhances the binding affinity of eukaryotic initiation factor 4F and (iso)4F for  cap analogues.	bind
7349	2	2661	7	10	NULL	0	NULL	(iso)4F	GP		binds					cap analogues	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1678_2_67_s_1026	15157733	(A) binding protein  enhances the binding affinity of eukaryotic initiation factor 4F and (iso)4F for  cap analogues.	bind
7350	3	2661	7	10	NULL	0	NULL	4F	GP		is a type of					eukaryotic initiation factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1678_2_67_s_1026	15157733	(A) binding protein  enhances the binding affinity of eukaryotic initiation factor 4F and (iso)4F for  cap analogues.	bind
7351	4	2661	7	10	NULL	0	NULL	(iso)4F	GP		is a type of					eukaryotic initiation factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1678_2_67_s_1026	15157733	(A) binding protein  enhances the binding affinity of eukaryotic initiation factor 4F and (iso)4F for  cap analogues.	bind
5305	1	2662	5	10	NULL	0	NULL	PABP	GP		bind					PCBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_6_1439_s_161	11250909	(A) binding protein (PABP) and poly(rC) binding protein (PCBP) interact with each other and the ends of the viral RNA to form a circular RNP complex.	bind
5306	2	2662	5	10	NULL	0	NULL	PCBP	GP		is					poly(rC) binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_6_1439_s_161	11250909	(A) binding protein (PABP) and poly(rC) binding protein (PCBP) interact with each other and the ends of the viral RNA to form a circular RNP complex.	bind
5307	3	2662	5	10	NULL	0	NULL	PABP	GP		bind					viral RNA	NucleicAcid		ends of		NULL		NULL	NULL	NULL	NULL	gw60_embo_20_6_1439_s_161	11250909	(A) binding protein (PABP) and poly(rC) binding protein (PCBP) interact with each other and the ends of the viral RNA to form a circular RNP complex.	bind
5308	4	2662	5	10	NULL	0	NULL	PCBP	GP		bind					viral RNA	NucleicAcid		ends of		NULL		NULL	NULL	NULL	NULL	gw60_embo_20_6_1439_s_161	11250909	(A) binding protein (PABP) and poly(rC) binding protein (PCBP) interact with each other and the ends of the viral RNA to form a circular RNP complex.	bind
5309	5	2662	5	10	NULL	0	NULL	statement 1	Process		forms					RNP complex	GP	circular			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_6_1439_s_161	11250909	(A) binding protein (PABP) and poly(rC) binding protein (PCBP) interact with each other and the ends of the viral RNA to form a circular RNP complex.	bind
5310	6	2662	5	10	NULL	0	NULL	statement 3	Process		forms					RNP complex	GP	circular 			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_6_1439_s_161	11250909	(A) binding protein (PABP) and poly(rC) binding protein (PCBP) interact with each other and the ends of the viral RNA to form a circular RNP complex.	bind
5311	7	2662	5	10	NULL	0	NULL	statement 4	Process		forms					RNP complex	GP	circular 			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_6_1439_s_161	11250909	(A) binding protein (PABP) and poly(rC) binding protein (PCBP) interact with each other and the ends of the viral RNA to form a circular RNP complex.	bind
5320	8	2662	5	10	NULL	0	NULL	PABP	GP		is					poly (A) binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_6_1439_s_161	11250909	(A) binding protein (PABP) and poly(rC) binding protein (PCBP) interact with each other and the ends of the viral RNA to form a circular RNP complex.	bind
7352	1	2662	7	10	NULL	0	NULL	PABP	GP		binds					PCBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_6_1439_s_161	11250909	(A) binding protein (PABP) and poly(rC) binding protein (PCBP) interact with each other and the ends of the viral RNA to form a circular RNP complex.	bind
7353	2	2662	7	10	NULL	0	NULL	PABP	GP		is					poly (A) binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_6_1439_s_161	11250909	(A) binding protein (PABP) and poly(rC) binding protein (PCBP) interact with each other and the ends of the viral RNA to form a circular RNP complex.	bind
7354	3	2662	7	10	NULL	0	NULL	PCBP	GP		is					poly(rC) binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_6_1439_s_161	11250909	(A) binding protein (PABP) and poly(rC) binding protein (PCBP) interact with each other and the ends of the viral RNA to form a circular RNP complex.	bind
7355	4	2662	7	10	NULL	0	NULL	PABP	GP		binds					Viral RNA	NucleicAcid		ends of		NULL		NULL	NULL	NULL	NULL	gw60_embo_20_6_1439_s_161	11250909	(A) binding protein (PABP) and poly(rC) binding protein (PCBP) interact with each other and the ends of the viral RNA to form a circular RNP complex.	bind
7356	5	2662	7	10	NULL	0	NULL	PCBP	GP		binds					Viral RNA	NucleicAcid		ends of		NULL		NULL	NULL	NULL	NULL	gw60_embo_20_6_1439_s_161	11250909	(A) binding protein (PABP) and poly(rC) binding protein (PCBP) interact with each other and the ends of the viral RNA to form a circular RNP complex.	bind
7357	6	2662	7	10	NULL	0	NULL	statement 1	Process		forms					RNP complex	GP	circular			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_6_1439_s_161	11250909	(A) binding protein (PABP) and poly(rC) binding protein (PCBP) interact with each other and the ends of the viral RNA to form a circular RNP complex.	bind
7358	7	2662	7	10	NULL	0	NULL	statement 4	Process		forms					RNP complex	GP	circular			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_6_1439_s_161	11250909	(A) binding protein (PABP) and poly(rC) binding protein (PCBP) interact with each other and the ends of the viral RNA to form a circular RNP complex.	bind
7359	8	2662	7	10	NULL	0	NULL	statement 5	Process		forms					RNP complex	GP	circular			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_6_1439_s_161	11250909	(A) binding protein (PABP) and poly(rC) binding protein (PCBP) interact with each other and the ends of the viral RNA to form a circular RNP complex.	bind
5312	1	2663	5	10	NULL	0	NULL	PABP	GP		bind					eIF4G	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4277_s_31	16705177	(A) binding protein (PABP); PABP also binds eIF4G.	bind
5321	2	2663	5	10	NULL	0	NULL	PABP	GP		is					poly (A) binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4277_s_31	16705177	(A) binding protein (PABP); PABP also binds eIF4G.	bind
7360	1	2663	7	10	NULL	0	NULL	PABP	GP		binds					eIF4G	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4277_s_31	16705177	(A) binding protein (PABP); PABP also binds eIF4G.	bind
7361	2	2663	7	10	NULL	0	NULL	PABP	GP		is					poly (A) binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4277_s_31	16705177	(A) binding protein (PABP); PABP also binds eIF4G.	bind
5313	1	2664	5	10	NULL	0	NULL	protein C1	GP		bind					pre-mRNA	NucleicAcid	nuclear			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_mol-cell-biol_26_8_16581783_s_1	16581783	(A) binding protein C1 binds nuclear pre-mRNA poly	bind
7876	1	2664	7	10	NULL	0	NULL	Protein C1	GP		binds					pre-mRNA	NucleicAcid	nuclear			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_mol-cell-biol_26_8_16581783_s_1	16581783	(A) binding protein C1 binds nuclear pre-mRNA poly	bind
5314	1	2668	5	10	NULL	0	NULL	Pab1	GP		bind					Dcp1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_16_4372_s_42	10944120	(A) binding protein Pab1 bind to Dcp1, either independently, or when these proteins are in the 5'' - 3' translation complex involving eIF4F and Pab1.	bind
5315	2	2668	5	10	NULL	0	NULL	statement 1	Process		occur					independently					NULL		NULL	NULL	NULL	NULL	gw60_embo_19_16_4372_s_42	10944120	(A) binding protein Pab1 bind to Dcp1, either independently, or when these proteins are in the 5'' - 3' translation complex involving eIF4F and Pab1.	bind
5316	3	2668	5	10	NULL	0	NULL	statement 1	Process		occurs in complex with					eIF4F	GP	5'' - 3' translation complex			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_16_4372_s_42	10944120	(A) binding protein Pab1 bind to Dcp1, either independently, or when these proteins are in the 5'' - 3' translation complex involving eIF4F and Pab1.	bind
5317	4	2668	5	10	NULL	0	NULL	statement 1	Process		occurs in complex with					Pab1	GP	5'' - 3' translation complex			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_16_4372_s_42	10944120	(A) binding protein Pab1 bind to Dcp1, either independently, or when these proteins are in the 5'' - 3' translation complex involving eIF4F and Pab1.	bind
5318	5	2668	5	10	NULL	0	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_16_4372_s_42	10944120	(A) binding protein Pab1 bind to Dcp1, either independently, or when these proteins are in the 5'' - 3' translation complex involving eIF4F and Pab1.	bind
5319	6	2668	5	10	NULL	0	NULL	statement 2	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_16_4372_s_42	10944120	(A) binding protein Pab1 bind to Dcp1, either independently, or when these proteins are in the 5'' - 3' translation complex involving eIF4F and Pab1.	bind
7362	1	2668	7	10	NULL	0	NULL	Pab1	GP		binds					Dcp1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_16_4372_s_42	10944120	(A) binding protein Pab1 bind to Dcp1, either independently, or when these proteins are in the 5'' - 3' translation complex involving eIF4F and Pab1.	bind
7363	2	2668	7	10	NULL	0	NULL	statement 1	Process		occurs					independently					NULL		NULL	NULL	NULL	NULL	gw60_embo_19_16_4372_s_42	10944120	(A) binding protein Pab1 bind to Dcp1, either independently, or when these proteins are in the 5'' - 3' translation complex involving eIF4F and Pab1.	bind
7364	3	2668	7	10	NULL	0	NULL	statement 1	Process		occurs in complex with					eIF4F	GP	5'' - 3' translation complex			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_16_4372_s_42	10944120	(A) binding protein Pab1 bind to Dcp1, either independently, or when these proteins are in the 5'' - 3' translation complex involving eIF4F and Pab1.	bind
7365	4	2668	7	10	NULL	0	NULL	statement 1	Process		occurs in complex with					Pab1	GP	5'' - 3' translation complex			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_16_4372_s_42	10944120	(A) binding protein Pab1 bind to Dcp1, either independently, or when these proteins are in the 5'' - 3' translation complex involving eIF4F and Pab1.	bind
8075	5	2668	7	10	NULL	0	NULL	statement 3	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_16_4372_s_42	10944120	(A) binding protein Pab1 bind to Dcp1, either independently, or when these proteins are in the 5'' - 3' translation complex involving eIF4F and Pab1.	bind
8076	6	2668	7	10	NULL	0	NULL	statement 4	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_16_4372_s_42	10944120	(A) binding protein Pab1 bind to Dcp1, either independently, or when these proteins are in the 5'' - 3' translation complex involving eIF4F and Pab1.	bind
5322	1	2669	5	10	NULL	0	NULL	RCC1	GP	endogenous	bind					mitotic chromosomes	Chromosome				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_160_5_635_s_155	12604592	(A) Both RanGDP and RanT24N strongly stimulate the binding of the endogenous RCC1  in the egg extract to the mitotic chromosomes assembled from the sperm chromatin.	bind
5323	2	2669	5	10	NULL	0	NULL	RanGDP	GP		stimulate		strongly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_160_5_635_s_155	12604592	(A) Both RanGDP and RanT24N strongly stimulate the binding of the endogenous RCC1  in the egg extract to the mitotic chromosomes assembled from the sperm chromatin.	bind
5324	3	2669	5	10	NULL	0	NULL	RanT24N	GP		stimulate		strongly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_160_5_635_s_155	12604592	(A) Both RanGDP and RanT24N strongly stimulate the binding of the endogenous RCC1  in the egg extract to the mitotic chromosomes assembled from the sperm chromatin.	bind
54140	4	2669	5	10	NULL	0	NULL	RCC1	GP		is from					egg extract	Cell				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_160_5_635_s_155	12604592	(A) Both RanGDP and RanT24N strongly stimulate the binding of the endogenous RCC1  in the egg extract to the mitotic chromosomes assembled from the sperm chromatin.	bind
54141	5	2669	5	10	NULL	0	NULL	mitotic chromosomes	Chromosome		are assembled from					sperm chromatin	Chromosome				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_160_5_635_s_155	12604592	(A) Both RanGDP and RanT24N strongly stimulate the binding of the endogenous RCC1  in the egg extract to the mitotic chromosomes assembled from the sperm chromatin.	bind
7366	1	2669	7	10	NULL	0	NULL	RCC1	GP	 endogenous	binds					mitotic chromosomes	Chromosome				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_160_5_635_s_155	12604592	(A) Both RanGDP and RanT24N strongly stimulate the binding of the endogenous RCC1  in the egg extract to the mitotic chromosomes assembled from the sperm chromatin.	bind
7367	2	2669	7	10	NULL	0	NULL	RCC1	GP		is from					egg extract	Cell				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_160_5_635_s_155	12604592	(A) Both RanGDP and RanT24N strongly stimulate the binding of the endogenous RCC1  in the egg extract to the mitotic chromosomes assembled from the sperm chromatin.	bind
7368	3	2669	7	10	NULL	0	NULL	mitotic chromosomes	Chromosome		are assembled from					sperm chromatin	Chromosome				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_160_5_635_s_155	12604592	(A) Both RanGDP and RanT24N strongly stimulate the binding of the endogenous RCC1  in the egg extract to the mitotic chromosomes assembled from the sperm chromatin.	bind
7369	4	2669	7	10	NULL	0	NULL	RanGDP	GP		stimulate		strongly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_160_5_635_s_155	12604592	(A) Both RanGDP and RanT24N strongly stimulate the binding of the endogenous RCC1  in the egg extract to the mitotic chromosomes assembled from the sperm chromatin.	bind
7370	5	2669	7	10	NULL	0	NULL	RanT24N	GP		stimulate		strongly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_160_5_635_s_155	12604592	(A) Both RanGDP and RanT24N strongly stimulate the binding of the endogenous RCC1  in the egg extract to the mitotic chromosomes assembled from the sperm chromatin.	bind
5325	1	2670	5	10	NULL	0	NULL	APP	GP		bind		directly	C terminus		KLC	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_28_2_449_s_126	11144355	(A) C terminus of APP directly binds KLC.	bind
7371	1	2670	7	10	NULL	0	NULL	APP	GP		binds		directly	C terminus		KLC	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_28_2_449_s_126	11144355	(A) C terminus of APP directly binds KLC.	bind
5326	1	2671	5	10	NULL	0	NULL	C1 bacteriophage	Organism		bind					cell wall	CellComponent	group C streptococcus			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_11_3325_s_84	12754230	(A) C1 bacteriophage binding to the cell wall of a group C streptococcus.	bind
7372	1	2671	7	10	NULL	0	NULL	C1 bacteriophage	Organism		binds to					cell wall	CellComponent	group C streptococcus			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_11_3325_s_84	12754230	(A) C1 bacteriophage binding to the cell wall of a group C streptococcus.	bind
5327	1	2672	5	NULL	NULL	0	NULL		NULL		bind	NULL		C644G			NULL			GRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8146_s_301	10567540	(A) C644G can bind to a GRE by EMSA.	bind
7373	1	2672	7	NULL	NULL	0	NULL		NULL		bind	NULL		C644G			NULL			GRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8146_s_301	10567540	(A) C644G can bind to a GRE by EMSA.	bind
5328	1	2673	5	10	NULL	0	NULL	syntaxin	GP		bind					synaptotagmin	GP		C2A domain		NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_86_1_39_s_129	9692742	(A) Ca2+-dependent syntaxin binding to synaptotagmin C2A domain.	bind
46340	2	2673	5	10	NULL	0	NULL	statement 1	GP		is dependent on					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_86_1_39_s_129	9692742	(A) Ca2+-dependent syntaxin binding to synaptotagmin C2A domain.	bind
7374	1	2673	7	10	NULL	0	NULL	syntaxin	GP		binds to					synaptotagmin	GP		C2A domain		NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_86_1_39_s_129	9692742	(A) Ca2+-dependent syntaxin binding to synaptotagmin C2A domain.	bind
46341	2	2673	7	10	NULL	0	NULL	statement 1	GP		is dependent on					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_86_1_39_s_129	9692742	(A) Ca2+-dependent syntaxin binding to synaptotagmin C2A domain.	bind
5330	1	2674	5	10	NULL	0	NULL	CAT	GP		bind					SHP2	GP				NULL	A549 cells	NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_89	15556604	(A) CAT binds SHP2 in A549 cells after FBS-stimulation.	bind
5331	2	2674	5	10	NULL	0	NULL	statement 1	GP		occurs after					FBS	Chemical	stimulation			NULL	A549 cells \t	NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_89	15556604	(A) CAT binds SHP2 in A549 cells after FBS-stimulation.	bind
7375	1	2674	7	10	NULL	0	NULL	 CAT	GP		binds					SHP2	GP				NULL	A549 cells	NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_89	15556604	(A) CAT binds SHP2 in A549 cells after FBS-stimulation.	bind
7376	2	2674	7	10	NULL	0	NULL	statement 1	Process		occurs after					FBS	Chemical	stimulation by			NULL	A549 cells \t	NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_89	15556604	(A) CAT binds SHP2 in A549 cells after FBS-stimulation.	bind
5332	1	2675	5	10	NULL	0	NULL	CAT	GP		bind					SHP2	GP				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_102	15556604	(A) CAT binds SHP2 upon stimulation of HeLa cells with FBS or fibrinogen,  while herbimycin-A and peptides comprising fibronectin functional sequence suppress  the biding.	bind
5333	2	2675	5	10	NULL	0	NULL	HeLa cells	Cell		is stimulated with					FBS	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_102	15556604	(A) CAT binds SHP2 upon stimulation of HeLa cells with FBS or fibrinogen,  while herbimycin-A and peptides comprising fibronectin functional sequence suppress  the biding.	bind
5334	3	2675	5	10	NULL	0	NULL	HeLa cells	Cell		is stimulated with					fibrinogen	GP				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_102	15556604	(A) CAT binds SHP2 upon stimulation of HeLa cells with FBS or fibrinogen,  while herbimycin-A and peptides comprising fibronectin functional sequence suppress  the biding.	bind
5335	4	2675	5	10	NULL	0	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_102	15556604	(A) CAT binds SHP2 upon stimulation of HeLa cells with FBS or fibrinogen,  while herbimycin-A and peptides comprising fibronectin functional sequence suppress  the biding.	bind
5336	5	2675	5	10	NULL	0	NULL	statement 2	Process		is required for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_102	15556604	(A) CAT binds SHP2 upon stimulation of HeLa cells with FBS or fibrinogen,  while herbimycin-A and peptides comprising fibronectin functional sequence suppress  the biding.	bind
5337	6	2675	5	10	NULL	0	NULL	statement 3	Process		is required for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_102	15556604	(A) CAT binds SHP2 upon stimulation of HeLa cells with FBS or fibrinogen,  while herbimycin-A and peptides comprising fibronectin functional sequence suppress  the biding.	bind
5338	7	2675	5	10	NULL	0	NULL	statement 5	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_102	15556604	(A) CAT binds SHP2 upon stimulation of HeLa cells with FBS or fibrinogen,  while herbimycin-A and peptides comprising fibronectin functional sequence suppress  the biding.	bind
5339	8	2675	5	10	NULL	0	NULL	herbimycin-A	Chemical		supress					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_102	15556604	(A) CAT binds SHP2 upon stimulation of HeLa cells with FBS or fibrinogen,  while herbimycin-A and peptides comprising fibronectin functional sequence suppress  the biding.	bind
5340	9	2675	5	10	NULL	0	NULL	statement 10	Process		supress					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_102	15556604	(A) CAT binds SHP2 upon stimulation of HeLa cells with FBS or fibrinogen,  while herbimycin-A and peptides comprising fibronectin functional sequence suppress  the biding.	bind
54236	10	2675	5	10	NULL	0	NULL	peptides	AminoAcid		comprise					fibronectin	GP	functional sequence			NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_102	15556604	(A) CAT binds SHP2 upon stimulation of HeLa cells with FBS or fibrinogen,  while herbimycin-A and peptides comprising fibronectin functional sequence suppress  the biding.	bind
7377	1	2675	7	10	NULL	0	NULL	CAT	GP		binds					SHP2	GP				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_102	15556604	(A) CAT binds SHP2 upon stimulation of HeLa cells with FBS or fibrinogen,  while herbimycin-A and peptides comprising fibronectin functional sequence suppress  the biding.	bind
7378	2	2675	7	10	NULL	0	NULL	HeLa cells	Cell		stimulated with					FBS	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_102	15556604	(A) CAT binds SHP2 upon stimulation of HeLa cells with FBS or fibrinogen,  while herbimycin-A and peptides comprising fibronectin functional sequence suppress  the biding.	bind
7379	3	2675	7	10	NULL	0	NULL	HeLa cells	Cell		stimulated with					fibrinogen	GP				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_102	15556604	(A) CAT binds SHP2 upon stimulation of HeLa cells with FBS or fibrinogen,  while herbimycin-A and peptides comprising fibronectin functional sequence suppress  the biding.	bind
7380	4	2675	7	10	NULL	0	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_102	15556604	(A) CAT binds SHP2 upon stimulation of HeLa cells with FBS or fibrinogen,  while herbimycin-A and peptides comprising fibronectin functional sequence suppress  the biding.	bind
7381	5	2675	7	10	NULL	0	NULL	statement 1	Process		occurs upon					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_102	15556604	(A) CAT binds SHP2 upon stimulation of HeLa cells with FBS or fibrinogen,  while herbimycin-A and peptides comprising fibronectin functional sequence suppress  the biding.	bind
54241	6	2675	7	10	NULL	0	NULL	herbimycin-A	Chemical		suppress					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_102	15556604	(A) CAT binds SHP2 upon stimulation of HeLa cells with FBS or fibrinogen,  while herbimycin-A and peptides comprising fibronectin functional sequence suppress  the biding.	bind
54242	7	2675	7	10	NULL	0	NULL	peptides	AminoAcid		comprise					fibronectin	GP	functional sequence			NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_102	15556604	(A) CAT binds SHP2 upon stimulation of HeLa cells with FBS or fibrinogen,  while herbimycin-A and peptides comprising fibronectin functional sequence suppress  the biding.	bind
54243	8	2675	7	10	NULL	0	NULL	statement 7	Process		suppress					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_102	15556604	(A) CAT binds SHP2 upon stimulation of HeLa cells with FBS or fibrinogen,  while herbimycin-A and peptides comprising fibronectin functional sequence suppress  the biding.	bind
5341	1	2677	5	10	NULL	0	NULL	ICP-1	GP	CBD-tagged	does not bind					CSC-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_161_2_229_s_131	12707312	(A) CBD-tagged ICP-1  does not bind to CSC-1 and binds weakly to BIR-1.	bind
5342	2	2677	5	10	NULL	0	NULL	ICP-1	GP	CBD-tagged	bind		weakly			BIR-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_161_2_229_s_131	12707312	(A) CBD-tagged ICP-1  does not bind to CSC-1 and binds weakly to BIR-1.	bind
7388	1	2677	7	10	NULL	0	NULL	ICP-1	GP	CBD-tagged	does not bind					CSC-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_161_2_229_s_131	12707312	(A) CBD-tagged ICP-1  does not bind to CSC-1 and binds weakly to BIR-1.	bind
7389	2	2677	7	10	NULL	0	NULL	ICP-1	GP	CBD-tagged	binds		weakly			BIR-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_161_2_229_s_131	12707312	(A) CBD-tagged ICP-1  does not bind to CSC-1 and binds weakly to BIR-1.	bind
5343	1	2679	5	10	NULL	0	NULL	Cdc24p	GP		bind					Gbeta	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_144_6_1187_s_265	10087263	(A) Cdc24p binds Gbeta in the presence of  MBPFar1.	bind
5344	2	2679	5	10	NULL	0	NULL	statement 1	Process		in the presence of					MBPFar1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_144_6_1187_s_265	10087263	(A) Cdc24p binds Gbeta in the presence of  MBPFar1.	bind
7390	1	2679	7	10	NULL	0	NULL	Cdc24p	GP		binds					Gbeta	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_144_6_1187_s_265	10087263	(A) Cdc24p binds Gbeta in the presence of  MBPFar1.	bind
7391	2	2679	7	10	NULL	0	NULL	statement 1	Process		occurs in the presence of					MBPFar1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_144_6_1187_s_265	10087263	(A) Cdc24p binds Gbeta in the presence of  MBPFar1.	bind
5345	1	2680	5	10	NULL	0	NULL	Cdc28	GP		bind					Cln2-deltaN-Sic1 fusions	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4463_s_266	12052857	(A) Cdc28 binds to Cln2-deltaN-Sic1 fusions.	bind
7392	1	2680	7	10	NULL	0	NULL	Cdc28	GP		binds					Cln2-deltaN-Sic1 fusions	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4463_s_266	12052857	(A) Cdc28 binds to Cln2-deltaN-Sic1 fusions.	bind
5346	1	2681	5	10	NULL	0	NULL	Cdc42Hs	GP		bind		spontaneously	F28L		GTP- -35S	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_10_794_s_18	9368762	(a) Cdc42Hs(F28L) spontaneously binds GTP-  -35S.	bind
7393	1	2681	7	10	NULL	0	NULL	Cdc42Hs	GP		binds		spontaneously	F28L		GTP- -35S	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_10_794_s_18	9368762	(a) Cdc42Hs(F28L) spontaneously binds GTP-  -35S.	bind
5347	1	2682	5	10	NULL	0	NULL	CDP/Cux	GP		bind					DNA pol alpha gene	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_3013_s_296	12665598	(A) CDP/Cux  binds to the DNA pol alpha gene promoter in vivo.	bind
7394	1	2682	7	10	NULL	0	NULL	CDP/Cux	GP		binds to					DNA pol alpha	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_3013_s_296	12665598	(A) CDP/Cux  binds to the DNA pol alpha gene promoter in vivo.	bind
5349	1	2686	5	10	NULL	0	NULL	CtIP	GP	cell-free;; synthesized	bind		specifically			GST-CtBP1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10379_s_214	16287852	(A) Cell-free synthesized  CtIP binds specifically to GST-CtBP1 (lane 2) and GST-SHARP-RD (lane 3) but not to  GST-RBP-2N (lane 1).	bind
5350	2	2686	5	10	NULL	0	NULL	CtIP	GP	cell-free;; synthesized	bind		specifically			GST-SHARP	GP		RD		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10379_s_214	16287852	(A) Cell-free synthesized  CtIP binds specifically to GST-CtBP1 (lane 2) and GST-SHARP-RD (lane 3) but not to  GST-RBP-2N (lane 1).	bind
5351	3	2686	5	10	NULL	0	NULL	CtIP	GP	cell-free;; synthesized	does not bind					GST-RBP	GP		2N		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10379_s_214	16287852	(A) Cell-free synthesized  CtIP binds specifically to GST-CtBP1 (lane 2) and GST-SHARP-RD (lane 3) but not to  GST-RBP-2N (lane 1).	bind
7395	1	2686	7	10	NULL	0	NULL	CtIP	GP	Cell-free;; synthesized	binds		specifically			GST-CtBP1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10379_s_214	16287852	(A) Cell-free synthesized  CtIP binds specifically to GST-CtBP1 (lane 2) and GST-SHARP-RD (lane 3) but not to  GST-RBP-2N (lane 1).	bind
7396	2	2686	7	10	NULL	0	NULL	CtIP	GP	Cell-free;; synthesized	binds		specifically			GST-SHARP	GP		RD		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10379_s_214	16287852	(A) Cell-free synthesized  CtIP binds specifically to GST-CtBP1 (lane 2) and GST-SHARP-RD (lane 3) but not to  GST-RBP-2N (lane 1).	bind
7397	3	2686	7	10	NULL	0	NULL	CtIP	GP	Cell-free;; synthesized	does not bind					GST-RBP	GP		2N		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10379_s_214	16287852	(A) Cell-free synthesized  CtIP binds specifically to GST-CtBP1 (lane 2) and GST-SHARP-RD (lane 3) but not to  GST-RBP-2N (lane 1).	bind
5861	1	2687	5	10	NULL	0	NULL	GTP	Chemical		bind					Ras	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_5_2807_s_227	12429740	(A) cells    ells were cultured for 24 h in the absence or presence of 1 muM dexamethasone; cell extracts were subjected to immunoprecipitation using the pan-Ras antibody   Y13259, and GTP and GTP + GDP bound to Ras were determined as described under	bind
5862	2	2687	5	10	NULL	0	NULL	GTP + GDP	Chemical		bind					Ras	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_5_2807_s_227	12429740	(A) cells    ells were cultured for 24 h in the absence or presence of 1 muM dexamethasone; cell extracts were subjected to immunoprecipitation using the pan-Ras antibody   Y13259, and GTP and GTP + GDP bound to Ras were determined as described under	bind
7398	1	2687	7	10	NULL	0	NULL	GTP	Chemical		binds to					Ras	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_5_2807_s_227	12429740	(A) cells    ells were cultured for 24 h in the absence or presence of 1 muM dexamethasone; cell extracts were subjected to immunoprecipitation using the pan-Ras antibody   Y13259, and GTP and GTP + GDP bound to Ras were determined as described under	bind
7399	2	2687	7	10	NULL	0	NULL	GTP + GDP	Chemical		binds to					Ras	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_5_2807_s_227	12429740	(A) cells    ells were cultured for 24 h in the absence or presence of 1 muM dexamethasone; cell extracts were subjected to immunoprecipitation using the pan-Ras antibody   Y13259, and GTP and GTP + GDP bound to Ras were determined as described under	bind
7240	1	2688	5	10	NULL	0	NULL	Ras 	GP	signaling of	activate		directly			Rho	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_5_2807_s_185	12429740	(A) Cells and NIH 3T3 Cells Transiently Transfected with Wild Type and Activated Ras-- Rho proteins are required for Ras-induced transformation, but there are conflicting data concerning whether Ras signaling directly causes Rho activation or whether some changes in Rho activity occur only during the selection of Ras-transformed cells  ( 5,  8,  16,  18,  23).	bind
7241	2	2688	5	10	NULL	0	NULL	Rho activity	Process	changes in	occur during					Ras-transformed cells	Cell	selection of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_5_2807_s_185	12429740	(A) Cells and NIH 3T3 Cells Transiently Transfected with Wild Type and Activated Ras-- Rho proteins are required for Ras-induced transformation, but there are conflicting data concerning whether Ras signaling directly causes Rho activation or whether some changes in Rho activity occur only during the selection of Ras-transformed cells  ( 5,  8,  16,  18,  23).	bind
7242	3	2688	5	10	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_5_2807_s_185	12429740	(A) Cells and NIH 3T3 Cells Transiently Transfected with Wild Type and Activated Ras-- Rho proteins are required for Ras-induced transformation, but there are conflicting data concerning whether Ras signaling directly causes Rho activation or whether some changes in Rho activity occur only during the selection of Ras-transformed cells  ( 5,  8,  16,  18,  23).	bind
7403	1	2688	7	10	NULL	0	NULL	Ras 	GP	signaling of	activate		directly			Rho	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_5_2807_s_185	12429740	(A) Cells and NIH 3T3 Cells Transiently Transfected with Wild Type and Activated Ras-- Rho proteins are required for Ras-induced transformation, but there are conflicting data concerning whether Ras signaling directly causes Rho activation or whether some changes in Rho activity occur only during the selection of Ras-transformed cells  ( 5,  8,  16,  18,  23).	bind
7404	2	2688	7	10	NULL	0	NULL	Rho activity	Process	changes in	occur during					Ras-transformed cells 	Cell	selection of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_5_2807_s_185	12429740	(A) Cells and NIH 3T3 Cells Transiently Transfected with Wild Type and Activated Ras-- Rho proteins are required for Ras-induced transformation, but there are conflicting data concerning whether Ras signaling directly causes Rho activation or whether some changes in Rho activity occur only during the selection of Ras-transformed cells  ( 5,  8,  16,  18,  23).	bind
7877	3	2688	7	10	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_5_2807_s_185	12429740	(A) Cells and NIH 3T3 Cells Transiently Transfected with Wild Type and Activated Ras-- Rho proteins are required for Ras-induced transformation, but there are conflicting data concerning whether Ras signaling directly causes Rho activation or whether some changes in Rho activity occur only during the selection of Ras-transformed cells  ( 5,  8,  16,  18,  23).	bind
5352	1	2691	5	10	NULL	0	NULL	Ssb1/2p	GP		bind					HSF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_5_1739_s_268	10793148	(A) Cells were grown in 5% glucose to prevent the binding of Ssb1/2p to HSF under normal growth conditions.	bind
7405	1	2691	7	10	NULL	0	NULL	Ssb1/2p	GP		binds					HSF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_5_1739_s_268	10793148	(A) Cells were grown in 5% glucose to prevent the binding of Ssb1/2p to HSF under normal growth conditions.	bind
5355	1	2692	5	10	NULL	0	NULL	nuclear proteins	GP		bind					IL-8 gene	GP			NF-kappaB binding site	NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_8_3872_s_167	10417151	(A) Characterization of nuclear proteins bound to the NF-kappaB binding site of the IL-8 gene.	bind
7407	1	2692	7	10	NULL	0	NULL	nuclear proteins	GP		binds to					IL-8 gene	GP			NF-kappaB binding site	NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_8_3872_s_167	10417151	(A) Characterization of nuclear proteins bound to the NF-kappaB binding site of the IL-8 gene.	bind
5356	1	2693	5	10	NULL	0	NULL	Smad1	GP		bind									I-BRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6646_s_335	12944489	(A) ChIP of Smad1 bound to I-BRE and BRE-1.	bind
5357	2	2693	5	10	NULL	0	NULL	Smad1	GP		bind									BRE-1	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6646_s_335	12944489	(A) ChIP of Smad1 bound to I-BRE and BRE-1.	bind
7408	1	2693	7	10	NULL	0	NULL	Smad1	GP		binds									I-BRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6646_s_335	12944489	(A) ChIP of Smad1 bound to I-BRE and BRE-1.	bind
7409	2	2693	7	10	NULL	0	NULL	Smad1	GP		binds									BRE-1	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6646_s_335	12944489	(A) ChIP of Smad1 bound to I-BRE and BRE-1.	bind
5358	1	2694	5	10	NULL	0	NULL	Smad1	GP		bind									I-BRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6646_s_224	12944489	(A) ChIP of Smad1 bound to I-BRE.	bind
7410	1	2694	7	10	NULL	0	NULL	Smad1	GP		binds to									I-BRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6646_s_224	12944489	(A) ChIP of Smad1 bound to I-BRE.	bind
5359	1	2695	5	10	NULL	0	NULL	HBP1	GP		bind					p47phox gene	GP	endogenous			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_7_3011_s_247	15024088	(A) ChIPs were used to test the binding of HBP1 to the endogenous p47phox gene.	bind
7411	1	2695	7	10	NULL	0	NULL	HBP1	GP		binds					p47phox gene	GP	endogenous			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_7_3011_s_247	15024088	(A) ChIPs were used to test the binding of HBP1 to the endogenous p47phox gene.	bind
5360	1	2697	5	10	NULL	0	NULL	E2F1	GP		bind					PPAR 1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_1_39_s_105	12110166	(A) Chromatin immunoprecipitation (ChIP) assays demonstrating binding of E2F1 and E2F4 to the  PPAR 1 promoter.	bind
5361	2	2697	5	10	NULL	0	NULL	E2F4	GP		bind					PPAR 1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_1_39_s_105	12110166	(A) Chromatin immunoprecipitation (ChIP) assays demonstrating binding of E2F1 and E2F4 to the  PPAR 1 promoter.	bind
7412	1	2697	7	10	NULL	0	NULL	E2F1	GP		binds					PPAR 1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_1_39_s_105	12110166	(A) Chromatin immunoprecipitation (ChIP) assays demonstrating binding of E2F1 and E2F4 to the  PPAR 1 promoter.	bind
7413	2	2697	7	10	NULL	0	NULL	E2F4	GP		binds					PPAR 1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_1_39_s_105	12110166	(A) Chromatin immunoprecipitation (ChIP) assays demonstrating binding of E2F1 and E2F4 to the  PPAR 1 promoter.	bind
5362	1	2698	5	10	NULL	0	NULL	NF-Y	GP		bind					ODF gene	GP	mouse			NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_1_512_s_124	15601870	(A) Chromatin immunoprecipitation analysis of NF-Y binding to the  mouse ODF gene in vivo.	bind
7414	1	2698	7	10	NULL	0	NULL	NF-Y	GP		binds					ODF gene	GP	mouse			NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_1_512_s_124	15601870	(A) Chromatin immunoprecipitation analysis of NF-Y binding to the  mouse ODF gene in vivo.	bind
5363	1	2699	5	10	NULL	0	NULL	Bet1	GP		bind			LxxLE sequence 		Sec23/24 complex	GP		B site		NULL		NULL	NULL	NULL	NULL	gw60_cell_114_4_483_s_60	12941276	(A) Close-up view of the Bet1 LxxLE sequence bound to the B site of the Sec23/24 complex.	bind
7415	1	2699	7	10	NULL	0	NULL	Bet1	GP		binds to			LxxLE sequence		Sec23/24 complex	GP		B site of 		NULL		NULL	NULL	NULL	NULL	gw60_cell_114_4_483_s_60	12941276	(A) Close-up view of the Bet1 LxxLE sequence bound to the B site of the Sec23/24 complex.	bind
5364	1	2700	5	10	NULL	0	NULL	EDA isoforms	GP		bind					EDAR receptors	GP				NULL		NULL	NULL	NULL	NULL	gw70_gene_371_1_42_s_107	16423472	(A) Co-immunoprecipitation analysis  for binding of EDA isoforms to EDAR, XEDAR, or TROY receptors.	bind
5365	2	2700	5	10	NULL	0	NULL	EDA isoforms	GP		bind					XEDAR receptors	GP				NULL		NULL	NULL	NULL	NULL	gw70_gene_371_1_42_s_107	16423472	(A) Co-immunoprecipitation analysis  for binding of EDA isoforms to EDAR, XEDAR, or TROY receptors.	bind
5366	3	2700	5	10	NULL	0	NULL	EDA isoforms	GP		bind					TROY receptors	GP				NULL		NULL	NULL	NULL	NULL	gw70_gene_371_1_42_s_107	16423472	(A) Co-immunoprecipitation analysis  for binding of EDA isoforms to EDAR, XEDAR, or TROY receptors.	bind
5367	4	2700	5	10	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_gene_371_1_42_s_107	16423472	(A) Co-immunoprecipitation analysis  for binding of EDA isoforms to EDAR, XEDAR, or TROY receptors.	bind
5368	5	2700	5	10	NULL	0	NULL	statement 1	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_gene_371_1_42_s_107	16423472	(A) Co-immunoprecipitation analysis  for binding of EDA isoforms to EDAR, XEDAR, or TROY receptors.	bind
5369	6	2700	5	10	NULL	0	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_gene_371_1_42_s_107	16423472	(A) Co-immunoprecipitation analysis  for binding of EDA isoforms to EDAR, XEDAR, or TROY receptors.	bind
7944	1	2700	7	10	NULL	0	NULL	EDA isoforms	GP		bind					EDAR receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_gene_371_1_42_s_107	16423472	(A) Co-immunoprecipitation analysis  for binding of EDA isoforms to EDAR, XEDAR, or TROY receptors.	bind
7945	2	2700	7	10	NULL	0	NULL	EDA isoforms	GP		bind					XEDAR receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_gene_371_1_42_s_107	16423472	(A) Co-immunoprecipitation analysis  for binding of EDA isoforms to EDAR, XEDAR, or TROY receptors.	bind
7946	3	2700	7	10	NULL	0	NULL	EDA isoforms	GP		bind					TROY receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_gene_371_1_42_s_107	16423472	(A) Co-immunoprecipitation analysis  for binding of EDA isoforms to EDAR, XEDAR, or TROY receptors.	bind
54143	4	2700	7	10	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_gene_371_1_42_s_107	16423472	(A) Co-immunoprecipitation analysis  for binding of EDA isoforms to EDAR, XEDAR, or TROY receptors.	bind
54144	5	2700	7	10	NULL	0	NULL	statement 1	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_gene_371_1_42_s_107	16423472	(A) Co-immunoprecipitation analysis  for binding of EDA isoforms to EDAR, XEDAR, or TROY receptors.	bind
54145	6	2700	7	10	NULL	0	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_gene_371_1_42_s_107	16423472	(A) Co-immunoprecipitation analysis  for binding of EDA isoforms to EDAR, XEDAR, or TROY receptors.	bind
5371	1	2701	5	10	NULL	0	NULL	Vav	GP		bind					SLP-76	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_2_155_s_88	9047237	(A) Coexpression of ZAP-70 induces binding between Vav and SLP-76.	bind
5373	2	2701	5	10	NULL	0	NULL	ZAP-70	GP	coexpression of	induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_2_155_s_88	9047237	(A) Coexpression of ZAP-70 induces binding between Vav and SLP-76.	bind
7947	1	2701	7	10	NULL	0	NULL	Vav	GP		bind					SLP-76	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_2_155_s_88	9047237	(A) Coexpression of ZAP-70 induces binding between Vav and SLP-76.	bind
7948	2	2701	7	10	NULL	0	NULL	ZAP-70	GP	coexpression of 	induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_2_155_s_88	9047237	(A) Coexpression of ZAP-70 induces binding between Vav and SLP-76.	bind
5375	1	2702	5	10	NULL	0	NULL	Rad24	GP		bind					Rfc5	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5485_s_252	9710632	(A) Coimmunoprecipitation of Rad24 and Rfc2 with Rfc5.	bind
5376	2	2702	5	10	NULL	0	NULL	Rfc2	GP		bind					Rfc5	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5485_s_252	9710632	(A) Coimmunoprecipitation of Rad24 and Rfc2 with Rfc5.	bind
7949	1	2702	7	10	NULL	0	NULL	Rad24	GP		bind					Rfc5	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5485_s_252	9710632	(A) Coimmunoprecipitation of Rad24 and Rfc2 with Rfc5.	bind
7950	2	2702	7	10	NULL	0	NULL	Rfc2	GP		bind					Rfc5	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5485_s_252	9710632	(A) Coimmunoprecipitation of Rad24 and Rfc2 with Rfc5.	bind
7243	1	2703	5	10	NULL	0	NULL	C3d	GP		bind		covalently			CD19 & Ag-IgM	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_2_107_s_218	9047233	(A) Coligation of CD19 and the Ag-receptor complex (IgM) by C3d covalently bound to Ag amplifies B cell responses.	bind
7244	2	2703	5	10	NULL	0	NULL	Ag-IgM	GP		is					Ag-receptor complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_2_107_s_218	9047233	(A) Coligation of CD19 and the Ag-receptor complex (IgM) by C3d covalently bound to Ag amplifies B cell responses.	bind
7245	3	2703	5	10	NULL	0	NULL	C3d	GP		coligates					CD19 & Ag-IgM	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_2_107_s_218	9047233	(A) Coligation of CD19 and the Ag-receptor complex (IgM) by C3d covalently bound to Ag amplifies B cell responses.	bind
7246	4	2703	5	10	NULL	0	NULL	statement 3	Process		amplifies					B cell responses	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_2_107_s_218	9047233	(A) Coligation of CD19 and the Ag-receptor complex (IgM) by C3d covalently bound to Ag amplifies B cell responses.	bind
7951	1	2703	7	10	NULL	0	NULL	C3d 	GP		bind		covalently			Ag	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_2_107_s_218	9047233	(A) Coligation of CD19 and the Ag-receptor complex (IgM) by C3d covalently bound to Ag amplifies B cell responses.	bind
7952	2	2703	7	10	NULL	0	NULL	statement 1	Process		coligates					CD19 & Ag-IgM	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_2_107_s_218	9047233	(A) Coligation of CD19 and the Ag-receptor complex (IgM) by C3d covalently bound to Ag amplifies B cell responses.	bind
7953	3	2703	7	10	NULL	0	NULL	Ag-IgM	GP		is					Ag-receptor complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_2_107_s_218	9047233	(A) Coligation of CD19 and the Ag-receptor complex (IgM) by C3d covalently bound to Ag amplifies B cell responses.	bind
7954	4	2703	7	10	NULL	0	NULL	statement 2	Process		amplifies					B cell responses	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_2_107_s_218	9047233	(A) Coligation of CD19 and the Ag-receptor complex (IgM) by C3d covalently bound to Ag amplifies B cell responses.	bind
5451	1	2707	5	10	NULL	0	NULL	histidine	AminoAcid		bind					hemes	Chemical				NULL	R. gelatinosus	NULL	NULL	NULL	NULL	gw60_jbacteriol_184_14_3815_s_153	12081951	(A) Comparison of the helix IV sequences showing the two histidines that bind the hemes (shaded) and the extra residue (boldface and underlined) in the  R. gelatinosus sequence.	bind
5452	2	2707	5	10	NULL	0	NULL	histidine	AminoAcid		bind					extra residue					NULL	R. gelatinosus	NULL	NULL	NULL	NULL	gw60_jbacteriol_184_14_3815_s_153	12081951	(A) Comparison of the helix IV sequences showing the two histidines that bind the hemes (shaded) and the extra residue (boldface and underlined) in the  R. gelatinosus sequence.	bind
7956	1	2707	7	10	NULL	0	NULL	histidine	AminoAcid		bind					hemes	Chemical				NULL	in R. gelatinosus	NULL	NULL	NULL	NULL	gw60_jbacteriol_184_14_3815_s_153	12081951	(A) Comparison of the helix IV sequences showing the two histidines that bind the hemes (shaded) and the extra residue (boldface and underlined) in the  R. gelatinosus sequence.	bind
7957	2	2707	7	10	NULL	0	NULL	histidines	AminoAcid		bind					extra residue					NULL	in R. gelatinosus	NULL	NULL	NULL	NULL	gw60_jbacteriol_184_14_3815_s_153	12081951	(A) Comparison of the helix IV sequences showing the two histidines that bind the hemes (shaded) and the extra residue (boldface and underlined) in the  R. gelatinosus sequence.	bind
5465	1	2709	5	10	NULL	0	NULL	GTP S	Chemical		bind					membranes	CellComponent	limbic forebrain			NULL	control mice	NULL	NULL	NULL	NULL	gw60_neuroscience_117_3_639_s_104	12617968	(A) Comparison of the stimulation of [35]GTP S binding by dopamine to membranes of the limbic forebrain obtained from control (B0: square) and BPA-treated (B2: triangle) mice.	bind
5467	2	2709	5	10	NULL	0	NULL	GTP S	Chemical		bind					membranes	CellComponent	limbic forebrain			NULL	BPA-treated mice	NULL	NULL	NULL	NULL	gw60_neuroscience_117_3_639_s_104	12617968	(A) Comparison of the stimulation of [35]GTP S binding by dopamine to membranes of the limbic forebrain obtained from control (B0: square) and BPA-treated (B2: triangle) mice.	bind
5469	3	2709	5	10	NULL	0	NULL	dopamine	Chemical		stimulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_117_3_639_s_104	12617968	(A) Comparison of the stimulation of [35]GTP S binding by dopamine to membranes of the limbic forebrain obtained from control (B0: square) and BPA-treated (B2: triangle) mice.	bind
5470	4	2709	5	10	NULL	0	NULL	dopamine	Chemical		stimulate					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_117_3_639_s_104	12617968	(A) Comparison of the stimulation of [35]GTP S binding by dopamine to membranes of the limbic forebrain obtained from control (B0: square) and BPA-treated (B2: triangle) mice.	bind
7958	1	2709	7	10	NULL	0	NULL	GTP S	Chemical		bind					membranes	CellComponent	limbic forebrain			NULL	in control mice	NULL	NULL	NULL	NULL	gw60_neuroscience_117_3_639_s_104	12617968	(A) Comparison of the stimulation of [35]GTP S binding by dopamine to membranes of the limbic forebrain obtained from control (B0: square) and BPA-treated (B2: triangle) mice.	bind
7959	2	2709	7	10	NULL	0	NULL	GTP S	Chemical		bind					 membranes	CellComponent	limbic forebrain			NULL	in BPA-treated mice	NULL	NULL	NULL	NULL	gw60_neuroscience_117_3_639_s_104	12617968	(A) Comparison of the stimulation of [35]GTP S binding by dopamine to membranes of the limbic forebrain obtained from control (B0: square) and BPA-treated (B2: triangle) mice.	bind
8851	3	2709	7	10	NULL	0	NULL	dopamine	Chemical		stimulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_117_3_639_s_104	12617968	(A) Comparison of the stimulation of [35]GTP S binding by dopamine to membranes of the limbic forebrain obtained from control (B0: square) and BPA-treated (B2: triangle) mice.	bind
8852	4	2709	7	10	NULL	0	NULL	dopamine	Chemical		stimulate					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_117_3_639_s_104	12617968	(A) Comparison of the stimulation of [35]GTP S binding by dopamine to membranes of the limbic forebrain obtained from control (B0: square) and BPA-treated (B2: triangle) mice.	bind
5472	1	2710	5	10	NULL	0	NULL	AP-1	GP		bind					AP-1 probe	NucleicAcid	unlabeled			NULL		NULL	NULL	NULL	NULL	gw60_brainres_872_1_282_s_78	10924710	(A) Competition of AP-1 binding with unlabeled AP-1 probe.	bind
7960	1	2710	7	10	NULL	0	NULL	AP-1	GP		bind					AP-1 probe	NucleicAcid	unlabeled			NULL		NULL	NULL	NULL	NULL	gw60_brainres_872_1_282_s_78	10924710	(A) Competition of AP-1 binding with unlabeled AP-1 probe.	bind
5473	1	2711	5	10	NULL	0	NULL	complex			bind					(eIF)-4G	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_17_4723_s_36	10970864	(A) complex binds to the translation factor eukaryotic initiation factor (eIF)-4G, which in turn interacts with eIF-4E bound to the cap ( Tarun and Sachs, 1996).	bind
5474	2	2711	5	10	NULL	0	NULL	(eIF)-4G	GP		is					translation factor eukaryotic initiation factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_17_4723_s_36	10970864	(A) complex binds to the translation factor eukaryotic initiation factor (eIF)-4G, which in turn interacts with eIF-4E bound to the cap ( Tarun and Sachs, 1996).	bind
5475	3	2711	5	10	NULL	0	NULL	eIF-4E	GP		bind					cap	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_17_4723_s_36	10970864	(A) complex binds to the translation factor eukaryotic initiation factor (eIF)-4G, which in turn interacts with eIF-4E bound to the cap ( Tarun and Sachs, 1996).	bind
5476	4	2711	5	10	NULL	0	NULL	statement 1	Process		interact with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_17_4723_s_36	10970864	(A) complex binds to the translation factor eukaryotic initiation factor (eIF)-4G, which in turn interacts with eIF-4E bound to the cap ( Tarun and Sachs, 1996).	bind
7961	1	2711	7	10	NULL	0	NULL	complex			binds					 eIF-4G	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_17_4723_s_36	10970864	(A) complex binds to the translation factor eukaryotic initiation factor (eIF)-4G, which in turn interacts with eIF-4E bound to the cap ( Tarun and Sachs, 1996).	bind
7962	3	2711	7	10	NULL	0	NULL	statement 1	Process		bind					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_17_4723_s_36	10970864	(A) complex binds to the translation factor eukaryotic initiation factor (eIF)-4G, which in turn interacts with eIF-4E bound to the cap ( Tarun and Sachs, 1996).	bind
7963	2	2711	7	10	NULL	0	NULL	eIF-4E	GP		bind					cap	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_17_4723_s_36	10970864	(A) complex binds to the translation factor eukaryotic initiation factor (eIF)-4G, which in turn interacts with eIF-4E bound to the cap ( Tarun and Sachs, 1996).	bind
8853	4	2711	7	10	NULL	0	NULL	(eIF)-4G	GP		is					eukaryotic initiation factor 	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_17_4723_s_36	10970864	(A) complex binds to the translation factor eukaryotic initiation factor (eIF)-4G, which in turn interacts with eIF-4E bound to the cap ( Tarun and Sachs, 1996).	bind
5479	1	2712	5	10	NULL	0	NULL	Kap121p	GP	recombinant	bind					GST-Ste12p	GP		aa494-688		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_8_2544_s_269	11909949	(A) Complexes containing recombinant Kap121p bound to GST-Ste12p (aa494-688) and immobilized on GT-Sepharose were incubated with Ran-GTP ( 120 ng), Ran-GDP ( 120 ng), or GTP-loading buffer, as indicated, for 30 min at room temperature.	bind
8069	1	2712	7	10	NULL	0	NULL	Kap121p	GP	recombinant	bind					GST-Ste12p	GP		aa 494-688		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_8_2544_s_269	11909949	(A) Complexes containing recombinant Kap121p bound to GST-Ste12p (aa494-688) and immobilized on GT-Sepharose were incubated with Ran-GTP ( 120 ng), Ran-GDP ( 120 ng), or GTP-loading buffer, as indicated, for 30 min at room temperature.	bind
5484	1	2714	5	10	NULL	0	NULL	HSV-1 capsids	CellComponent	isolated	bind					liver nuclei	CellComponent	purified;; rat			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4922_s_203	10848617	(A) Confocal immunofluorescence microscopy of isolated HSV-1 capsids bound to purified rat liver nuclei in the presence of rat liver cytosol (control panel).	bind
5486	2	2714	5	10	NULL	0	NULL	statement 1	Process		in the presence of					liver cytosol 	CellComponent	rat			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4922_s_203	10848617	(A) Confocal immunofluorescence microscopy of isolated HSV-1 capsids bound to purified rat liver nuclei in the presence of rat liver cytosol (control panel).	bind
8070	1	2714	7	10	NULL	0	NULL	HSV-1 capsids	CellComponent	isolated	bind					liver nuclei	CellComponent	purified;; rat 			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4922_s_203	10848617	(A) Confocal immunofluorescence microscopy of isolated HSV-1 capsids bound to purified rat liver nuclei in the presence of rat liver cytosol (control panel).	bind
46396	2	2714	7	10	NULL	0	NULL	statement 1	Process		occurs in presence of					liver cytosol	CellComponent	rat			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4922_s_203	10848617	(A) Confocal immunofluorescence microscopy of isolated HSV-1 capsids bound to purified rat liver nuclei in the presence of rat liver cytosol (control panel).	bind
5488	1	2716	5	10	NULL	0	NULL	GFP-Ras isoforms	GP	constitutively;; active	bind		preferentially			GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_5_865_s_55	12021258	(A) Constitutively active GFP-Ras isoforms preferentially bind GTP.	bind
8071	1	2716	7	10	NULL	0	NULL	GFP-Ras isoforms	GP	Constitutively;; active	bind		preferentially			GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_5_865_s_55	12021258	(A) Constitutively active GFP-Ras isoforms preferentially bind GTP.	bind
5497	1	2722	5	10	NULL	0	NULL	Yrb1	GP		bind					GST-Gsp1GTP	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4295_s_216	10825193	(A) Cooperative binding of Yrb1 and Xpo1 to GST-Gsp1GTP.	bind
5498	2	2722	5	10	NULL	0	NULL	Xpo1	GP		bind					GST-Gsp1GTP	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4295_s_216	10825193	(A) Cooperative binding of Yrb1 and Xpo1 to GST-Gsp1GTP.	bind
5499	3	2722	5	10	NULL	0	NULL	statement 1	Process		occurs in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4295_s_216	10825193	(A) Cooperative binding of Yrb1 and Xpo1 to GST-Gsp1GTP.	bind
8072	1	2722	7	10	NULL	0	NULL	Yrb1	GP		bind					GST-Gsp1GTP	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4295_s_216	10825193	(A) Cooperative binding of Yrb1 and Xpo1 to GST-Gsp1GTP.	bind
8073	2	2722	7	10	NULL	0	NULL	Xpo1	GP		bind					GST-Gsp1GTP	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4295_s_216	10825193	(A) Cooperative binding of Yrb1 and Xpo1 to GST-Gsp1GTP.	bind
8096	3	2722	7	10	NULL	0	NULL	statement 1	Process		occurs in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4295_s_216	10825193	(A) Cooperative binding of Yrb1 and Xpo1 to GST-Gsp1GTP.	bind
5500	1	2723	5	10	NULL	0	NULL	Oct-1	GP		bind			POU domain		DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_14_4700_s_242	11416146	(A) Cooperative VP16 binding to the Oct-1 POU domain-DNA complex.	bind
5501	2	2723	5	10	NULL	0	NULL	VP16	GP		bind		cooperative			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_14_4700_s_242	11416146	(A) Cooperative VP16 binding to the Oct-1 POU domain-DNA complex.	bind
8097	1	2723	7	10	NULL	0	NULL	VP16 	GP		bind					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_14_4700_s_242	11416146	(A) Cooperative VP16 binding to the Oct-1 POU domain-DNA complex.	bind
8854	2	2723	7	10	NULL	0	NULL	Oct-1	GP		bind			POU		DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_14_4700_s_242	11416146	(A) Cooperative VP16 binding to the Oct-1 POU domain-DNA complex.	bind
5508	1	2725	5	10	NULL	0	NULL	CR2	GP		bind					Tax	GP	putative	transactivation domain		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_16_5520_s_222	11463834	(A) CR2 binds to the putative transactivation domain of Tax.	bind
8100	1	2725	7	10	NULL	0	NULL	 CR2	GP		bind					Tax	GP	putative 	transactivation domain		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_16_5520_s_222	11463834	(A) CR2 binds to the putative transactivation domain of Tax.	bind
5512	1	2726	5	10	NULL	0	NULL	OspB	GP		bind					CR3	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_9_6138_s_94	16113335	(A) CR3 clustering (red); (B) OspB binding superimposed  on CR3 (green).	bind
54148	1	2726	7	10	NULL	0	NULL	OspB	GP		bind					CR3	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_9_6138_s_94	16113335	(A) CR3 clustering (red); (B) OspB binding superimposed  on CR3 (green).	bind
5513	1	2727	5	10	NULL	0	NULL	p53	GP		bind					CBP	GP		KIX domain		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4849_s_87	10848610	(A) CREB enhances p53 binding to the KIX domain of CBP.	bind
5514	2	2727	5	10	NULL	0	NULL	CREB	GP		enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4849_s_87	10848610	(A) CREB enhances p53 binding to the KIX domain of CBP.	bind
8147	1	2727	7	10	NULL	0	NULL	p53	GP		binds					CBP	GP		KIX		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4849_s_87	10848610	(A) CREB enhances p53 binding to the KIX domain of CBP.	bind
8148	2	2727	7	10	NULL	0	NULL	CREB	GP		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4849_s_87	10848610	(A) CREB enhances p53 binding to the KIX domain of CBP.	bind
5515	1	2728	5	10	NULL	0	NULL	CRF	GP		bind					CRF receptor 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_30_4_513_s_140	16198122	(A) CRF binds to CRF receptor 1 to evoke protein kinase C-mediated signaling pathways  and cause a fine tuning state A of the common CRF and UCN signaling machinery (Sig  A).	bind
5517	2	2728	5	10	NULL	0	NULL	statement 1	Process		evoke					protein kinase C-mediated signaling pathways	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_30_4_513_s_140	16198122	(A) CRF binds to CRF receptor 1 to evoke protein kinase C-mediated signaling pathways  and cause a fine tuning state A of the common CRF and UCN signaling machinery (Sig  A).	bind
5519	3	2728	5	10	NULL	0	NULL	statement 1	Process		causes					common CRF signaling machinery	Process	fine tuning state A of 			NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_30_4_513_s_140	16198122	(A) CRF binds to CRF receptor 1 to evoke protein kinase C-mediated signaling pathways  and cause a fine tuning state A of the common CRF and UCN signaling machinery (Sig  A).	bind
9047	4	2728	5	10	NULL	0	NULL	statement 1	Process		causes					common UCN signaling machinery	Process	fine tuning state A of			NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_30_4_513_s_140	16198122	(A) CRF binds to CRF receptor 1 to evoke protein kinase C-mediated signaling pathways  and cause a fine tuning state A of the common CRF and UCN signaling machinery (Sig  A).	bind
8149	1	2728	7	10	NULL	0	NULL	CRF	GP		binds					CRF receptor 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_30_4_513_s_140	16198122	(A) CRF binds to CRF receptor 1 to evoke protein kinase C-mediated signaling pathways  and cause a fine tuning state A of the common CRF and UCN signaling machinery (Sig  A).	bind
8150	2	2728	7	10	NULL	0	NULL	statement 1	Process		evoke					protein kinase C-mediated signaling pathways	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_30_4_513_s_140	16198122	(A) CRF binds to CRF receptor 1 to evoke protein kinase C-mediated signaling pathways  and cause a fine tuning state A of the common CRF and UCN signaling machinery (Sig  A).	bind
8151	3	2728	7	10	NULL	0	NULL	statement 1	Process		cause					common CRF signaling machinery	Process	fine tuning state A of			NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_30_4_513_s_140	16198122	(A) CRF binds to CRF receptor 1 to evoke protein kinase C-mediated signaling pathways  and cause a fine tuning state A of the common CRF and UCN signaling machinery (Sig  A).	bind
8152	4	2728	7	10	NULL	0	NULL	statement 1	Process		cause					UCN signaling machinery 	Process	fine tuning state A of			NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_30_4_513_s_140	16198122	(A) CRF binds to CRF receptor 1 to evoke protein kinase C-mediated signaling pathways  and cause a fine tuning state A of the common CRF and UCN signaling machinery (Sig  A).	bind
5521	1	2729	5	10	NULL	0	NULL	CRP	GP		bind					Ppac	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_7_2215_s_89	15028709	(A) CRP binding to the  Ppac promoter.	bind
8163	1	2729	7	10	NULL	0	NULL	CRP	GP		binds					Ppac	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_7_2215_s_89	15028709	(A) CRP binding to the  Ppac promoter.	bind
5522	1	2730	5	10	NULL	0	NULL	CRT	GP		bind					NES	AminoAcid	WT			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_1_127_s_231	11149926	(A) CRT binding to the WT NES requires the presence of RanGTP.	bind
5524	2	2730	5	10	NULL	0	NULL	statement 1	Process		occurs in presence of					RanGTP	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_1_127_s_231	11149926	(A) CRT binding to the WT NES requires the presence of RanGTP.	bind
8280	1	2730	7	10	NULL	0	NULL	CRT	GP		binds					NES	AminoAcid	WT			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_1_127_s_231	11149926	(A) CRT binding to the WT NES requires the presence of RanGTP.	bind
8281	2	2730	7	10	NULL	0	NULL	statement 1	Process		occurs in the presence of					RanGTP	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_1_127_s_231	11149926	(A) CRT binding to the WT NES requires the presence of RanGTP.	bind
5527	1	2731	5	10	NULL	0	NULL	CtsR	GP		bind		specifically			clpB	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_4_1165_s_171	14762012	(A) CtsR binds specifically to the  clpB promoter region.	bind
8282	1	2731	7	10	NULL	0	NULL	CtsR	GP		bind		specifically			clpB	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_4_1165_s_171	14762012	(A) CtsR binds specifically to the  clpB promoter region.	bind
5528	1	2732	5	10	NULL	0	NULL	CtsR	GP		bind		specifically			clpP	GP	S. salivarius		promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_2_683_s_51	12511518	(A) CtsR binds specifically to the  S. salivarius clpP promoter region.	bind
8283	1	2732	7	10	NULL	0	NULL	CtsR	GP		bind		specifically			clpP	GP	S. salivarius		promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_2_683_s_51	12511518	(A) CtsR binds specifically to the  S. salivarius clpP promoter region.	bind
5530	1	2733	5	10	NULL	0	NULL	AgrA	GP		bind							isolated		P2 repeats	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_22_7549_s_149	15516566	(A) Curves showing binding of AgrA to isolated P2 and P3 repeats and to P3  mutant fragments.	bind
5532	2	2733	5	10	NULL	0	NULL	AgrA	GP		bind							isolated		P3 repeats	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_22_7549_s_149	15516566	(A) Curves showing binding of AgrA to isolated P2 and P3 repeats and to P3  mutant fragments.	bind
5533	3	2733	5	10	NULL	0	NULL	AgrA	GP		bind					P3 fragments	AminoAcid	mutant 			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_22_7549_s_149	15516566	(A) Curves showing binding of AgrA to isolated P2 and P3 repeats and to P3  mutant fragments.	bind
8284	1	2733	7	10	NULL	0	NULL	AgrA	GP		binds							isolated		P2 repeats	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_22_7549_s_149	15516566	(A) Curves showing binding of AgrA to isolated P2 and P3 repeats and to P3  mutant fragments.	bind
8285	2	2733	7	10	NULL	0	NULL	AgrA	GP		bind							isolated		P3 repeats	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_22_7549_s_149	15516566	(A) Curves showing binding of AgrA to isolated P2 and P3 repeats and to P3  mutant fragments.	bind
8286	3	2733	7	10	NULL	0	NULL	AgrA	GP		bind					P3 fragment	AminoAcid	mutant			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_22_7549_s_149	15516566	(A) Curves showing binding of AgrA to isolated P2 and P3 repeats and to P3  mutant fragments.	bind
5534	1	2735	5	10	NULL	0	NULL	Daam1	GP		bind					Dvl2	GP		PDZ domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_843_s_98	11779461	(A) Daam1  and C-Daam1 bind to the Dvl2 PDZ  and DEP domains, but not to the DIX  domain.	bind
5535	2	2735	5	10	NULL	0	NULL	Daam1	GP		bind					Dvl2	GP		DEP domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_843_s_98	11779461	(A) Daam1  and C-Daam1 bind to the Dvl2 PDZ  and DEP domains, but not to the DIX  domain.	bind
5537	3	2735	5	10	NULL	0	NULL	Daam1	GP		does not bind					Dvl2	GP		DIX domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_843_s_98	11779461	(A) Daam1  and C-Daam1 bind to the Dvl2 PDZ  and DEP domains, but not to the DIX  domain.	bind
5540	4	2735	5	10	NULL	0	NULL	C-Daam1	GP		bind					Dvl2	GP		PDZ domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_843_s_98	11779461	(A) Daam1  and C-Daam1 bind to the Dvl2 PDZ  and DEP domains, but not to the DIX  domain.	bind
5541	5	2735	5	10	NULL	0	NULL	C-Daam1	GP		bind					Dvl2	GP		DEP domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_843_s_98	11779461	(A) Daam1  and C-Daam1 bind to the Dvl2 PDZ  and DEP domains, but not to the DIX  domain.	bind
5542	6	2735	5	10	NULL	0	NULL	C-Daam1	GP		does not bind					Dvl2	GP		DIX domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_843_s_98	11779461	(A) Daam1  and C-Daam1 bind to the Dvl2 PDZ  and DEP domains, but not to the DIX  domain.	bind
8287	1	2735	7	10	NULL	0	NULL	Daam1	GP		bind					Dvl2	GP		PDZ		NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_843_s_98	11779461	(A) Daam1  and C-Daam1 bind to the Dvl2 PDZ  and DEP domains, but not to the DIX  domain.	bind
8288	2	2735	7	10	NULL	0	NULL	Daam1	GP		bind					Dvl2	GP		DEP		NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_843_s_98	11779461	(A) Daam1  and C-Daam1 bind to the Dvl2 PDZ  and DEP domains, but not to the DIX  domain.	bind
8289	3	2735	7	10	NULL	0	NULL	Daam1	GP		does not bind					Dvl2	GP		DIX		NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_843_s_98	11779461	(A) Daam1  and C-Daam1 bind to the Dvl2 PDZ  and DEP domains, but not to the DIX  domain.	bind
8290	4	2735	7	10	NULL	0	NULL	C-Daam1	GP		bind					Dvl2	GP		PDZ		NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_843_s_98	11779461	(A) Daam1  and C-Daam1 bind to the Dvl2 PDZ  and DEP domains, but not to the DIX  domain.	bind
8291	5	2735	7	10	NULL	0	NULL	C-Daam1	GP		bind					Dvl2	GP		DEP		NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_843_s_98	11779461	(A) Daam1  and C-Daam1 bind to the Dvl2 PDZ  and DEP domains, but not to the DIX  domain.	bind
8292	6	2735	7	10	NULL	0	NULL	C-Daam1	GP		does not bind					Dvl2	GP		DIX		NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_843_s_98	11779461	(A) Daam1  and C-Daam1 bind to the Dvl2 PDZ  and DEP domains, but not to the DIX  domain.	bind
5543	1	2736	5	10	NULL	0	NULL	SLP-76	GP		bind			SH2 domain		CD6P	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_17_6727_s_176	16914752	(A) Data for two concentrations (muM) of the  SLP-76 SH2 domain show binding to CD6P, weaker binding to 662F, and no binding to  CD6, where only the bulk effect of the high-protein concentration is seen.	bind
5544	2	2736	5	10	NULL	0	NULL	SLP-76	GP		bind		weakly	SH2 domain					662F		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_17_6727_s_176	16914752	(A) Data for two concentrations (muM) of the  SLP-76 SH2 domain show binding to CD6P, weaker binding to 662F, and no binding to  CD6, where only the bulk effect of the high-protein concentration is seen.	bind
5545	3	2736	5	10	NULL	0	NULL	SLP-76	GP		does not bind			SH2 domain		CD6	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_17_6727_s_176	16914752	(A) Data for two concentrations (muM) of the  SLP-76 SH2 domain show binding to CD6P, weaker binding to 662F, and no binding to  CD6, where only the bulk effect of the high-protein concentration is seen.	bind
8293	1	2736	7	10	NULL	0	NULL	SLP-76	GP		bind			SH2 domain		CD6P	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_17_6727_s_176	16914752	(A) Data for two concentrations (muM) of the  SLP-76 SH2 domain show binding to CD6P, weaker binding to 662F, and no binding to  CD6, where only the bulk effect of the high-protein concentration is seen.	bind
8294	2	2736	7	10	NULL	0	NULL	SLP-76	GP		bind		weakly	SH2 domain					662F		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_17_6727_s_176	16914752	(A) Data for two concentrations (muM) of the  SLP-76 SH2 domain show binding to CD6P, weaker binding to 662F, and no binding to  CD6, where only the bulk effect of the high-protein concentration is seen.	bind
8295	3	2736	7	10	NULL	0	NULL	SLP-76	GP		does not bind			SH2 domain		CD6	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_17_6727_s_176	16914752	(A) Data for two concentrations (muM) of the  SLP-76 SH2 domain show binding to CD6P, weaker binding to 662F, and no binding to  CD6, where only the bulk effect of the high-protein concentration is seen.	bind
5852	1	2737	5	10	NULL	0	NULL	DDR	GP		bind					collagens	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_129	9659900	(A) DDR binding to different types of commercially-derived collagens; note weaker binding of both DDR1 and DDR2 to network-forming collagen type IV as compared to rest of collagens, which are all examples of fibril-forming collagens (K, kangaroo tail; B, bovine nasal septum; C, calf skin; H, human placenta; R, rat tail; roman numerals represent biochemical types of collagen).	bind
5853	2	2737	5	10	NULL	0	NULL	DDR1	GP		bind					collagen type IV	GP	network-forming			NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_129	9659900	(A) DDR binding to different types of commercially-derived collagens; note weaker binding of both DDR1 and DDR2 to network-forming collagen type IV as compared to rest of collagens, which are all examples of fibril-forming collagens (K, kangaroo tail; B, bovine nasal septum; C, calf skin; H, human placenta; R, rat tail; roman numerals represent biochemical types of collagen).	bind
5854	3	2737	5	10	NULL	0	NULL	DDR2	GP		bind					collagen type IV	GP	network-forming			NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_129	9659900	(A) DDR binding to different types of commercially-derived collagens; note weaker binding of both DDR1 and DDR2 to network-forming collagen type IV as compared to rest of collagens, which are all examples of fibril-forming collagens (K, kangaroo tail; B, bovine nasal septum; C, calf skin; H, human placenta; R, rat tail; roman numerals represent biochemical types of collagen).	bind
5855	4	2737	5	10	NULL	0	NULL	DDR1	GP		bind					collagens	GP	fibril-forming			NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_129	9659900	(A) DDR binding to different types of commercially-derived collagens; note weaker binding of both DDR1 and DDR2 to network-forming collagen type IV as compared to rest of collagens, which are all examples of fibril-forming collagens (K, kangaroo tail; B, bovine nasal septum; C, calf skin; H, human placenta; R, rat tail; roman numerals represent biochemical types of collagen).	bind
5856	5	2737	5	10	NULL	0	NULL	DDR2	GP		bind					collagens	GP	fibril-forming			NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_129	9659900	(A) DDR binding to different types of commercially-derived collagens; note weaker binding of both DDR1 and DDR2 to network-forming collagen type IV as compared to rest of collagens, which are all examples of fibril-forming collagens (K, kangaroo tail; B, bovine nasal septum; C, calf skin; H, human placenta; R, rat tail; roman numerals represent biochemical types of collagen).	bind
5857	6	2737	5	10	NULL	0	NULL	statement 2	Process		weaker than					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_129	9659900	(A) DDR binding to different types of commercially-derived collagens; note weaker binding of both DDR1 and DDR2 to network-forming collagen type IV as compared to rest of collagens, which are all examples of fibril-forming collagens (K, kangaroo tail; B, bovine nasal septum; C, calf skin; H, human placenta; R, rat tail; roman numerals represent biochemical types of collagen).	bind
5858	7	2737	5	10	NULL	0	NULL	statement 2	Process		weaker than					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_129	9659900	(A) DDR binding to different types of commercially-derived collagens; note weaker binding of both DDR1 and DDR2 to network-forming collagen type IV as compared to rest of collagens, which are all examples of fibril-forming collagens (K, kangaroo tail; B, bovine nasal septum; C, calf skin; H, human placenta; R, rat tail; roman numerals represent biochemical types of collagen).	bind
5859	8	2737	5	10	NULL	0	NULL	statement 3	Process		weaker than					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_129	9659900	(A) DDR binding to different types of commercially-derived collagens; note weaker binding of both DDR1 and DDR2 to network-forming collagen type IV as compared to rest of collagens, which are all examples of fibril-forming collagens (K, kangaroo tail; B, bovine nasal septum; C, calf skin; H, human placenta; R, rat tail; roman numerals represent biochemical types of collagen).	bind
5860	9	2737	5	10	NULL	0	NULL	statement 3	Process		weaker than					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_129	9659900	(A) DDR binding to different types of commercially-derived collagens; note weaker binding of both DDR1 and DDR2 to network-forming collagen type IV as compared to rest of collagens, which are all examples of fibril-forming collagens (K, kangaroo tail; B, bovine nasal septum; C, calf skin; H, human placenta; R, rat tail; roman numerals represent biochemical types of collagen).	bind
8296	1	2737	7	10	NULL	0	NULL	DDR	GP		bind					collagen	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_129	9659900	(A) DDR binding to different types of commercially-derived collagens; note weaker binding of both DDR1 and DDR2 to network-forming collagen type IV as compared to rest of collagens, which are all examples of fibril-forming collagens (K, kangaroo tail; B, bovine nasal septum; C, calf skin; H, human placenta; R, rat tail; roman numerals represent biochemical types of collagen).	bind
8297	2	2737	7	10	NULL	0	NULL	DDR1	GP		bind		weakly			collagen type IV	GP	network forming			NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_129	9659900	(A) DDR binding to different types of commercially-derived collagens; note weaker binding of both DDR1 and DDR2 to network-forming collagen type IV as compared to rest of collagens, which are all examples of fibril-forming collagens (K, kangaroo tail; B, bovine nasal septum; C, calf skin; H, human placenta; R, rat tail; roman numerals represent biochemical types of collagen).	bind
8298	3	2737	7	10	NULL	0	NULL	DDR2	GP		bind		weakly			collagen type IV	GP	network forming			NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_129	9659900	(A) DDR binding to different types of commercially-derived collagens; note weaker binding of both DDR1 and DDR2 to network-forming collagen type IV as compared to rest of collagens, which are all examples of fibril-forming collagens (K, kangaroo tail; B, bovine nasal septum; C, calf skin; H, human placenta; R, rat tail; roman numerals represent biochemical types of collagen).	bind
9107	4	2737	7	10	NULL	0	NULL	DDR1	GP		bind					collagen	GP	fibril-forming			NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_129	9659900	(A) DDR binding to different types of commercially-derived collagens; note weaker binding of both DDR1 and DDR2 to network-forming collagen type IV as compared to rest of collagens, which are all examples of fibril-forming collagens (K, kangaroo tail; B, bovine nasal septum; C, calf skin; H, human placenta; R, rat tail; roman numerals represent biochemical types of collagen).	bind
9108	5	2737	7	10	NULL	0	NULL	DDR2	GP		bind					collagen	GP	fibril-forming			NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_129	9659900	(A) DDR binding to different types of commercially-derived collagens; note weaker binding of both DDR1 and DDR2 to network-forming collagen type IV as compared to rest of collagens, which are all examples of fibril-forming collagens (K, kangaroo tail; B, bovine nasal septum; C, calf skin; H, human placenta; R, rat tail; roman numerals represent biochemical types of collagen).	bind
9109	6	2737	7	10	NULL	0	NULL	statement 2	Process		is weaker than					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_129	9659900	(A) DDR binding to different types of commercially-derived collagens; note weaker binding of both DDR1 and DDR2 to network-forming collagen type IV as compared to rest of collagens, which are all examples of fibril-forming collagens (K, kangaroo tail; B, bovine nasal septum; C, calf skin; H, human placenta; R, rat tail; roman numerals represent biochemical types of collagen).	bind
9110	7	2737	7	10	NULL	0	NULL	statement 3	Process		is weaker than					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_129	9659900	(A) DDR binding to different types of commercially-derived collagens; note weaker binding of both DDR1 and DDR2 to network-forming collagen type IV as compared to rest of collagens, which are all examples of fibril-forming collagens (K, kangaroo tail; B, bovine nasal septum; C, calf skin; H, human placenta; R, rat tail; roman numerals represent biochemical types of collagen).	bind
5546	1	2739	5	10	NULL	0	NULL	Rac	GP		bind					GST-PAK-1	GP		CRIB domain		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_3_481_s_166	11980921	(A) Detection of Rac bound to the GST-PAK-1 CRIB domain after fibronectin adhesion for the given times.	bind
5547	2	2739	5	10	NULL	0	NULL	fibronectin adhesion	Process		is required for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_3_481_s_166	11980921	(A) Detection of Rac bound to the GST-PAK-1 CRIB domain after fibronectin adhesion for the given times.	bind
8299	1	2739	7	10	NULL	0	NULL	Rac	GP		bind					GST-PAK-1	GP		CRIB		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_3_481_s_166	11980921	(A) Detection of Rac bound to the GST-PAK-1 CRIB domain after fibronectin adhesion for the given times.	bind
8300	2	2739	7	10	NULL	0	NULL	statement 1	Process		occurs after					fibronectin adhesion	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_3_481_s_166	11980921	(A) Detection of Rac bound to the GST-PAK-1 CRIB domain after fibronectin adhesion for the given times.	bind
5548	1	2740	5	10	NULL	0	NULL	T10-TM	GP	in vitro-translated	bind		selectively			Enigma	GP		PDZ domain		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_6_1973_s_131	10359609	(A) Detergent extracts of skeletal beta-TM fusion protein (35S-T10-TM) generated by in vitro translation were probed with glutathione-agarose-coupled GST or GST-PDZ domains of Enigma, Dlg (PDZs 1 and 2), LIM kinase, and ENH. T10-TM binds selectively to the PDZ domain of Enigma.	bind
8313	1	2740	7	10	NULL	0	NULL	T10-TM 	GP	In vitro-translated	bind		selectively			Enigma	GP		PDZ		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_6_1973_s_131	10359609	(A) Detergent extracts of skeletal beta-TM fusion protein (35S-T10-TM) generated by in vitro translation were probed with glutathione-agarose-coupled GST or GST-PDZ domains of Enigma, Dlg (PDZs 1 and 2), LIM kinase, and ENH. T10-TM binds selectively to the PDZ domain of Enigma.	bind
5648	1	2742	5	10	NULL	0	NULL	HSF	GP		activate					hsp70	GP	Drosophila		promoter	NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_5_511_s_25	8805267	(a) Diagram of  Drosophila hsp70  preset  promoter before (top) and after (bottom) activation by heat-shock factor (HSF), which binds to the heat-shock elements (HSEs).	bind
5649	2	2742	5	10	NULL	0	NULL	HSF	GP		is					heat-shock factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_5_511_s_25	8805267	(a) Diagram of  Drosophila hsp70  preset  promoter before (top) and after (bottom) activation by heat-shock factor (HSF), which binds to the heat-shock elements (HSEs).	bind
5650	3	2742	5	10	NULL	0	NULL	hsp70	GP	Drosophila	bind				promoter	HSEs	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_5_511_s_25	8805267	(a) Diagram of  Drosophila hsp70  preset  promoter before (top) and after (bottom) activation by heat-shock factor (HSF), which binds to the heat-shock elements (HSEs).	bind
5651	4	2742	5	10	NULL	0	NULL	HSEs	NucleicAcid		is					heat-shock elements	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_5_511_s_25	8805267	(a) Diagram of  Drosophila hsp70  preset  promoter before (top) and after (bottom) activation by heat-shock factor (HSF), which binds to the heat-shock elements (HSEs).	bind
5652	5	2742	5	10	NULL	0	NULL	statement 3	Process		occurs before					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_5_511_s_25	8805267	(a) Diagram of  Drosophila hsp70  preset  promoter before (top) and after (bottom) activation by heat-shock factor (HSF), which binds to the heat-shock elements (HSEs).	bind
5653	6	2742	5	10	NULL	0	NULL	statement 3	Process		occurs after					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_5_511_s_25	8805267	(a) Diagram of  Drosophila hsp70  preset  promoter before (top) and after (bottom) activation by heat-shock factor (HSF), which binds to the heat-shock elements (HSEs).	bind
8314	1	2742	7	10	NULL	0	NULL	hsp70	GP	Drosophila	bind				preset promoter	HSEs	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_5_511_s_25	8805267	(a) Diagram of  Drosophila hsp70  preset  promoter before (top) and after (bottom) activation by heat-shock factor (HSF), which binds to the heat-shock elements (HSEs).	bind
8315	2	2742	7	10	NULL	0	NULL	HSEs	NucleicAcid		is					 heat-shock elements	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_5_511_s_25	8805267	(a) Diagram of  Drosophila hsp70  preset  promoter before (top) and after (bottom) activation by heat-shock factor (HSF), which binds to the heat-shock elements (HSEs).	bind
8316	3	2742	7	10	NULL	0	NULL	statement 1	Process		occurs before					HSF	GP	activation by			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_5_511_s_25	8805267	(a) Diagram of  Drosophila hsp70  preset  promoter before (top) and after (bottom) activation by heat-shock factor (HSF), which binds to the heat-shock elements (HSEs).	bind
8318	4	2742	7	10	NULL	0	NULL	statement 1	Process		occurs after					HSF	GP	activation by			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_5_511_s_25	8805267	(a) Diagram of  Drosophila hsp70  preset  promoter before (top) and after (bottom) activation by heat-shock factor (HSF), which binds to the heat-shock elements (HSEs).	bind
8320	5	2742	7	10	NULL	0	NULL	HSF	GP		is					heat-shock factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_5_511_s_25	8805267	(a) Diagram of  Drosophila hsp70  preset  promoter before (top) and after (bottom) activation by heat-shock factor (HSF), which binds to the heat-shock elements (HSEs).	bind
54149	6	2742	7	10	NULL	0	NULL	HSF	GP		activate					hsp70	GP	Drosophila		promoter	NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_5_511_s_25	8805267	(a) Diagram of  Drosophila hsp70  preset  promoter before (top) and after (bottom) activation by heat-shock factor (HSF), which binds to the heat-shock elements (HSEs).	bind
5654	1	2743	5	10	NULL	0	NULL	DIAP1	GP		bind					DCP-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_98_4_453_s_119	10481910	(A) DIAP1 binds DCP-1 and HID, and the first 37 residues of  HID are required for this interaction.	bind
5655	2	2743	5	10	NULL	0	NULL	DIAP1	GP		bind					HID	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_98_4_453_s_119	10481910	(A) DIAP1 binds DCP-1 and HID, and the first 37 residues of  HID are required for this interaction.	bind
5656	3	2743	5	10	NULL	0	NULL	HID	GP		is required for			first 37 residues		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_98_4_453_s_119	10481910	(A) DIAP1 binds DCP-1 and HID, and the first 37 residues of  HID are required for this interaction.	bind
8323	1	2743	7	10	NULL	0	NULL	DIAP1	GP		binds					DCP-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_98_4_453_s_119	10481910	(A) DIAP1 binds DCP-1 and HID, and the first 37 residues of  HID are required for this interaction.	bind
8325	2	2743	7	10	NULL	0	NULL	DIAP1 	GP		binds					HID	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_98_4_453_s_119	10481910	(A) DIAP1 binds DCP-1 and HID, and the first 37 residues of  HID are required for this interaction.	bind
8328	3	2743	7	10	NULL	0	NULL	statement 2	Process		requires					HID	GP		first 37 residues		NULL		NULL	NULL	NULL	NULL	gw60_cell_98_4_453_s_119	10481910	(A) DIAP1 binds DCP-1 and HID, and the first 37 residues of  HID are required for this interaction.	bind
5657	1	2744	5	10	NULL	0	NULL	C hnRNP protein	GP		bind					U2 snRNP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_40_24922_s_50	8798770	(A) did not compete for the binding of C hnRNP protein to U2 snRNP (Fig.  2,  lane 4).	bind
8332	1	2744	7	10	NULL	0	NULL	C hnRNP	GP		bind					U2 snRNP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_40_24922_s_50	8798770	(A) did not compete for the binding of C hnRNP protein to U2 snRNP (Fig.  2,  lane 4).	bind
5658	1	2745	5	10	NULL	0	NULL	C3G peptide	AminoAcid		bind					c-Crk	GP		SH3-N		NULL		NULL	NULL	NULL	NULL	gw60_structure_3_2_215_s_67	7735837	(a) Difference electron-density map for the C3G peptide bound to c-Crk SH3-N.	bind
8333	1	2745	7	10	NULL	0	NULL	C3G peptide	AminoAcid		bind					c-Crk	GP		SH3-N		NULL		NULL	NULL	NULL	NULL	gw60_structure_3_2_215_s_67	7735837	(a) Difference electron-density map for the C3G peptide bound to c-Crk SH3-N.	bind
5659	1	2746	5	10	NULL	0	NULL	laminin-2	GP	biotinylated	bind		directly			PGL-1	Chemical	native;; M. leprae			NULL		NULL	NULL	NULL	NULL	gw60_cell_103_3_511_s_102	11081637	(A) Direct binding of biotinylated  laminin-2 to native  M. leprae PGL-1 and its derivatives.	bind
5660	2	2746	5	10	NULL	0	NULL	laminin-2	GP	biotinylated	bind		directly			PGL-1 derivatives	Chemical	native;; M. leprae			NULL		NULL	NULL	NULL	NULL	gw60_cell_103_3_511_s_102	11081637	(A) Direct binding of biotinylated  laminin-2 to native  M. leprae PGL-1 and its derivatives.	bind
8335	1	2746	7	10	NULL	0	NULL	laminin-2	GP	biotinylated 	bind		directly			PGL-1	Chemical	native;; M. leprae			NULL		NULL	NULL	NULL	NULL	gw60_cell_103_3_511_s_102	11081637	(A) Direct binding of biotinylated  laminin-2 to native  M. leprae PGL-1 and its derivatives.	bind
8336	2	2746	7	10	NULL	0	NULL	laminin-2	GP	biotinylated 	bind		directly			PGL-1 derivatives	Chemical	native;; M. leprae			NULL		NULL	NULL	NULL	NULL	gw60_cell_103_3_511_s_102	11081637	(A) Direct binding of biotinylated  laminin-2 to native  M. leprae PGL-1 and its derivatives.	bind
5661	1	2747	5	10	NULL	0	NULL	125I- -bungarotoxin	Chemical		bind					SH-SY5Y-h 7 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_13_2533_s_126	11044725	(A) displacement of 125I- -bungarotoxin ( -BTx) binding to SH-SY5Y-h 7 cells by diltiazem.	bind
5662	2	2747	5	10	NULL	0	NULL	diltiazem	Chemical		bind					SH-SY5Y-h 7 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_13_2533_s_126	11044725	(A) displacement of 125I- -bungarotoxin ( -BTx) binding to SH-SY5Y-h 7 cells by diltiazem.	bind
5663	3	2747	5	10	NULL	0	NULL	statement 1	Process		is displaced by					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_13_2533_s_126	11044725	(A) displacement of 125I- -bungarotoxin ( -BTx) binding to SH-SY5Y-h 7 cells by diltiazem.	bind
46397	4	2747	5	10	NULL	0	NULL	BTx	Chemical		is					bungarotoxin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_13_2533_s_126	11044725	(A) displacement of 125I- -bungarotoxin ( -BTx) binding to SH-SY5Y-h 7 cells by diltiazem.	bind
8337	1	2747	7	10	NULL	0	NULL	125I- -bungarotoxin	Chemical		bind					SH-SY5Y-h 7 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_13_2533_s_126	11044725	(A) displacement of 125I- -bungarotoxin ( -BTx) binding to SH-SY5Y-h 7 cells by diltiazem.	bind
8338	2	2747	7	10	NULL	0	NULL	BTx	Chemical		is					bungarotoxin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_13_2533_s_126	11044725	(A) displacement of 125I- -bungarotoxin ( -BTx) binding to SH-SY5Y-h 7 cells by diltiazem.	bind
8340	3	2747	7	10	NULL	0	NULL	diltiazem	Chemical		bind					SH-SY5Y-h 7 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_13_2533_s_126	11044725	(A) displacement of 125I- -bungarotoxin ( -BTx) binding to SH-SY5Y-h 7 cells by diltiazem.	bind
8341	4	2747	7	10	NULL	0	NULL	diltiazem	Chemical		displaces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_13_2533_s_126	11044725	(A) displacement of 125I- -bungarotoxin ( -BTx) binding to SH-SY5Y-h 7 cells by diltiazem.	bind
5664	1	2748	5	10	NULL	0	NULL	RNAP	GP		bind					RNA:DNA hybrid	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_2_1_55_s_84	9702191	(A) Dissociation of the   subunit after binding of RNAP to the RNA:DNA hybrid.	bind
8343	1	2748	7	10	NULL	0	NULL	RNAP	GP		bind					RNA:DNA hybrid	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_2_1_55_s_84	9702191	(A) Dissociation of the   subunit after binding of RNAP to the RNA:DNA hybrid.	bind
5734	1	2749	5	10	NULL	0	NULL	p53	GP		bind					DNA	NucleicAcid			PG13	NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_683_s_92	11463392	(A) DNA binding activity of p53 to oligonucleotides containing two consensus p53 binding sites (PG13), PUMA binding site 1 (PUMA BS1), PUMA binding site 2 (PUMA BS2), and mutant PUMA binding site 2 (mt PUMA BS2).	bind
5736	2	2749	5	10	NULL	0	NULL	p53	GP		bind					oligonucleotides	NucleicAcid			PUMA BS1	NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_683_s_92	11463392	(A) DNA binding activity of p53 to oligonucleotides containing two consensus p53 binding sites (PG13), PUMA binding site 1 (PUMA BS1), PUMA binding site 2 (PUMA BS2), and mutant PUMA binding site 2 (mt PUMA BS2).	bind
5737	3	2749	5	10	NULL	0	NULL	PUMA BS1	NucleicAcid		is					PUMA binding site 1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_683_s_92	11463392	(A) DNA binding activity of p53 to oligonucleotides containing two consensus p53 binding sites (PG13), PUMA binding site 1 (PUMA BS1), PUMA binding site 2 (PUMA BS2), and mutant PUMA binding site 2 (mt PUMA BS2).	bind
5738	4	2749	5	10	NULL	0	NULL	p53	GP		bind					oligonucleotides	NucleicAcid			PUMA BS2	NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_683_s_92	11463392	(A) DNA binding activity of p53 to oligonucleotides containing two consensus p53 binding sites (PG13), PUMA binding site 1 (PUMA BS1), PUMA binding site 2 (PUMA BS2), and mutant PUMA binding site 2 (mt PUMA BS2).	bind
5739	5	2749	5	10	NULL	0	NULL	PUMA BS2	NucleicAcid		is					PUMA binding site 2	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_683_s_92	11463392	(A) DNA binding activity of p53 to oligonucleotides containing two consensus p53 binding sites (PG13), PUMA binding site 1 (PUMA BS1), PUMA binding site 2 (PUMA BS2), and mutant PUMA binding site 2 (mt PUMA BS2).	bind
5740	6	2749	5	10	NULL	0	NULL	p53	GP		bind					oligonucleotides	NucleicAcid			mt PUMA BS2	NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_683_s_92	11463392	(A) DNA binding activity of p53 to oligonucleotides containing two consensus p53 binding sites (PG13), PUMA binding site 1 (PUMA BS1), PUMA binding site 2 (PUMA BS2), and mutant PUMA binding site 2 (mt PUMA BS2).	bind
5741	7	2749	5	10	NULL	0	NULL	mt PUMA BS2	NucleicAcid		is					mutant PUMA binding site 2	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_683_s_92	11463392	(A) DNA binding activity of p53 to oligonucleotides containing two consensus p53 binding sites (PG13), PUMA binding site 1 (PUMA BS1), PUMA binding site 2 (PUMA BS2), and mutant PUMA binding site 2 (mt PUMA BS2).	bind
8365	1	2749	7	10	NULL	0	NULL	p53	GP		bind					DNA	NucleicAcid			PG13	NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_683_s_92	11463392	(A) DNA binding activity of p53 to oligonucleotides containing two consensus p53 binding sites (PG13), PUMA binding site 1 (PUMA BS1), PUMA binding site 2 (PUMA BS2), and mutant PUMA binding site 2 (mt PUMA BS2).	bind
8369	2	2749	7	10	NULL	0	NULL	p53	GP		bind					oligonucleotide	NucleicAcid			PUMA BS1	NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_683_s_92	11463392	(A) DNA binding activity of p53 to oligonucleotides containing two consensus p53 binding sites (PG13), PUMA binding site 1 (PUMA BS1), PUMA binding site 2 (PUMA BS2), and mutant PUMA binding site 2 (mt PUMA BS2).	bind
8372	3	2749	7	10	NULL	0	NULL	p53	GP		bind					oligonucleotide	NucleicAcid			PUMA BS2	NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_683_s_92	11463392	(A) DNA binding activity of p53 to oligonucleotides containing two consensus p53 binding sites (PG13), PUMA binding site 1 (PUMA BS1), PUMA binding site 2 (PUMA BS2), and mutant PUMA binding site 2 (mt PUMA BS2).	bind
8373	4	2749	7	10	NULL	0	NULL	p53	GP		bind					oligonucleotide	NucleicAcid			mt PUMA BS2	NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_683_s_92	11463392	(A) DNA binding activity of p53 to oligonucleotides containing two consensus p53 binding sites (PG13), PUMA binding site 1 (PUMA BS1), PUMA binding site 2 (PUMA BS2), and mutant PUMA binding site 2 (mt PUMA BS2).	bind
8374	5	2749	7	10	NULL	0	NULL	PG13	NucleicAcid		is					 p53 binding site	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_683_s_92	11463392	(A) DNA binding activity of p53 to oligonucleotides containing two consensus p53 binding sites (PG13), PUMA binding site 1 (PUMA BS1), PUMA binding site 2 (PUMA BS2), and mutant PUMA binding site 2 (mt PUMA BS2).	bind
8375	6	2749	7	10	NULL	0	NULL	PUMA BS1	NucleicAcid		is					PUMA binding site 1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_683_s_92	11463392	(A) DNA binding activity of p53 to oligonucleotides containing two consensus p53 binding sites (PG13), PUMA binding site 1 (PUMA BS1), PUMA binding site 2 (PUMA BS2), and mutant PUMA binding site 2 (mt PUMA BS2).	bind
8376	7	2749	7	10	NULL	0	NULL	PUMA BS2	NucleicAcid		is					PUMA binding site 2	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_683_s_92	11463392	(A) DNA binding activity of p53 to oligonucleotides containing two consensus p53 binding sites (PG13), PUMA binding site 1 (PUMA BS1), PUMA binding site 2 (PUMA BS2), and mutant PUMA binding site 2 (mt PUMA BS2).	bind
8377	8	2749	7	10	NULL	0	NULL	mt PUMA BS2	NucleicAcid		is					mutant PUMA binding site 2	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_683_s_92	11463392	(A) DNA binding activity of p53 to oligonucleotides containing two consensus p53 binding sites (PG13), PUMA binding site 1 (PUMA BS1), PUMA binding site 2 (PUMA BS2), and mutant PUMA binding site 2 (mt PUMA BS2).	bind
5742	1	2751	5	10	NULL	NULL	NULL	255 bp fragment	NucleicAcid		include					Race	GP	proximal region of		533 bp enhancer (349-533)	NULL		NULL	NULL	NULL	NULL	gw70_development_132_7_1637_s_164	15728670	(A) DNAse I footprinting analysis of Mad and Zen GST fusion proteins  bound to a 255 bp fragment that includes the proximal region of the  Race 533 bp enhancer (349-533) and 70 nucleotides from the Bluescript vector.	bind
5744	2	2751	5	10	NULL	NULL	NULL	255 bp fragment	NucleicAcid		include					70 nucleotides	NucleicAcid	from Bluescript vector			NULL		NULL	NULL	NULL	NULL	gw70_development_132_7_1637_s_164	15728670	(A) DNAse I footprinting analysis of Mad and Zen GST fusion proteins  bound to a 255 bp fragment that includes the proximal region of the  Race 533 bp enhancer (349-533) and 70 nucleotides from the Bluescript vector.	bind
5745	3	2751	5	10	NULL	NULL	NULL	Mad	GP		bind					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_132_7_1637_s_164	15728670	(A) DNAse I footprinting analysis of Mad and Zen GST fusion proteins  bound to a 255 bp fragment that includes the proximal region of the  Race 533 bp enhancer (349-533) and 70 nucleotides from the Bluescript vector.	bind
5747	4	2751	5	10	NULL	NULL	NULL	Zen	GP		bind					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_132_7_1637_s_164	15728670	(A) DNAse I footprinting analysis of Mad and Zen GST fusion proteins  bound to a 255 bp fragment that includes the proximal region of the  Race 533 bp enhancer (349-533) and 70 nucleotides from the Bluescript vector.	bind
54237	5	2751	5	10	NULL	NULL	NULL	statement 1	Process		occurs simultaneously with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_132_7_1637_s_164	15728670	(A) DNAse I footprinting analysis of Mad and Zen GST fusion proteins  bound to a 255 bp fragment that includes the proximal region of the  Race 533 bp enhancer (349-533) and 70 nucleotides from the Bluescript vector.	bind
54238	6	2751	5	10	NULL	NULL	NULL	Mad	GP		is a type of					GST fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_132_7_1637_s_164	15728670	(A) DNAse I footprinting analysis of Mad and Zen GST fusion proteins  bound to a 255 bp fragment that includes the proximal region of the  Race 533 bp enhancer (349-533) and 70 nucleotides from the Bluescript vector.	bind
54239	7	2751	5	10	NULL	NULL	NULL	Zen	GP		is a type of					GST fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_132_7_1637_s_164	15728670	(A) DNAse I footprinting analysis of Mad and Zen GST fusion proteins  bound to a 255 bp fragment that includes the proximal region of the  Race 533 bp enhancer (349-533) and 70 nucleotides from the Bluescript vector.	bind
8836	1	2751	7	10	NULL	NULL	NULL	255 bp fragment	NucleicAcid		contains					Race	GP			proximal region of  533 bp enhancer (349-533)	NULL		NULL	NULL	NULL	NULL	gw70_development_132_7_1637_s_164	15728670	(A) DNAse I footprinting analysis of Mad and Zen GST fusion proteins  bound to a 255 bp fragment that includes the proximal region of the  Race 533 bp enhancer (349-533) and 70 nucleotides from the Bluescript vector.	bind
8837	4	2751	7	10	NULL	NULL	NULL	Mad	GP		bind					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_132_7_1637_s_164	15728670	(A) DNAse I footprinting analysis of Mad and Zen GST fusion proteins  bound to a 255 bp fragment that includes the proximal region of the  Race 533 bp enhancer (349-533) and 70 nucleotides from the Bluescript vector.	bind
8838	3	2751	7	10	NULL	NULL	NULL	statement 1	Process		occur simultaneously with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_132_7_1637_s_164	15728670	(A) DNAse I footprinting analysis of Mad and Zen GST fusion proteins  bound to a 255 bp fragment that includes the proximal region of the  Race 533 bp enhancer (349-533) and 70 nucleotides from the Bluescript vector.	bind
8839	2	2751	7	10	NULL	NULL	NULL	255 bp fragment	NucleicAcid		contains					70 nucleotides 	NucleicAcid	  Bluescript vector			NULL		NULL	NULL	NULL	NULL	gw70_development_132_7_1637_s_164	15728670	(A) DNAse I footprinting analysis of Mad and Zen GST fusion proteins  bound to a 255 bp fragment that includes the proximal region of the  Race 533 bp enhancer (349-533) and 70 nucleotides from the Bluescript vector.	bind
54244	5	2751	7	10	NULL	NULL	NULL	Zen	GP		bind					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_132_7_1637_s_164	15728670	(A) DNAse I footprinting analysis of Mad and Zen GST fusion proteins  bound to a 255 bp fragment that includes the proximal region of the  Race 533 bp enhancer (349-533) and 70 nucleotides from the Bluescript vector.	bind
54245	6	2751	7	10	NULL	NULL	NULL	Mad	GP		is a type of					GST fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_132_7_1637_s_164	15728670	(A) DNAse I footprinting analysis of Mad and Zen GST fusion proteins  bound to a 255 bp fragment that includes the proximal region of the  Race 533 bp enhancer (349-533) and 70 nucleotides from the Bluescript vector.	bind
54246	7	2751	7	10	NULL	NULL	NULL	Zen	GP		is a type of					GST fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_132_7_1637_s_164	15728670	(A) DNAse I footprinting analysis of Mad and Zen GST fusion proteins  bound to a 255 bp fragment that includes the proximal region of the  Race 533 bp enhancer (349-533) and 70 nucleotides from the Bluescript vector.	bind
5748	1	2752	5	10	NULL	NULL	NULL	XylRdeltaA protein	GP		bind					Pu	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_cell_86_2_331_s_58	8706137	(A) DNase I footprints  caused by increasing amounts of XylRdeltaA protein (0, 0.1, 0.2, 0.4, 0.6, 0.8, and 1.0 muM) bound to the  Pu promoter in the presence or absence of 5 mM ATP.	bind
8840	1	2752	7	10	NULL	NULL	NULL	XylRdeltaA protein	GP		bind					Pu	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_cell_86_2_331_s_58	8706137	(A) DNase I footprints  caused by increasing amounts of XylRdeltaA protein (0, 0.1, 0.2, 0.4, 0.6, 0.8, and 1.0 muM) bound to the  Pu promoter in the presence or absence of 5 mM ATP.	bind
5752	1	2753	5	10	NULL	NULL	NULL	PtxS	GP		bind					ptxS	GP			upstream region	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_16_4890_s_190	10438759	(A) DNase I protection analysis of PtxS binding to the  ptxS upstream region.	bind
8841	1	2753	7	10	NULL	NULL	NULL	PtxS	GP		bind					ptxS	GP			 upstream region	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_16_4890_s_190	10438759	(A) DNase I protection analysis of PtxS binding to the  ptxS upstream region.	bind
5753	1	2754	5	10	NULL	NULL	NULL	DOKL	GP		bind					v-Abl	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8314_s_269	10567556	(A) DOKL binding to v-Abl requires Abl kinase activity and the DOKL PTB domain.	bind
5754	2	2754	5	10	NULL	NULL	NULL	Abl kinase 	GP	activity of	is required for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8314_s_269	10567556	(A) DOKL binding to v-Abl requires Abl kinase activity and the DOKL PTB domain.	bind
5755	3	2754	5	10	NULL	NULL	NULL	DOKL	GP		is required for			PTB domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8314_s_269	10567556	(A) DOKL binding to v-Abl requires Abl kinase activity and the DOKL PTB domain.	bind
8842	1	2754	7	10	NULL	NULL	NULL	DOKL	GP		bind					v-Abl	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8314_s_269	10567556	(A) DOKL binding to v-Abl requires Abl kinase activity and the DOKL PTB domain.	bind
8843	2	2754	7	10	NULL	NULL	NULL	statement 1	Process		requires					Abl kinase	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8314_s_269	10567556	(A) DOKL binding to v-Abl requires Abl kinase activity and the DOKL PTB domain.	bind
8844	3	2754	7	10	NULL	NULL	NULL	statement 1	Process		requires					DOKL 	GP		PTB		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8314_s_269	10567556	(A) DOKL binding to v-Abl requires Abl kinase activity and the DOKL PTB domain.	bind
5756	1	2755	5	10	NULL	NULL	NULL	Domain III proteins	GP		bind					E1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_1_111_s_189	16216925	(A) Domain III proteins bind to E1 during fusion.	bind
5757	2	2755	5	10	NULL	NULL	NULL	statement 1	Process		occurs during					fusion	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_1_111_s_189	16216925	(A) Domain III proteins bind to E1 during fusion.	bind
8845	1	2755	7	10	NULL	NULL	NULL	Domain III protein	GP		bind					E1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_1_111_s_189	16216925	(A) Domain III proteins bind to E1 during fusion.	bind
8846	2	2755	7	10	NULL	NULL	NULL	statement 1	Process		occurs during					fusion	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_1_111_s_189	16216925	(A) Domain III proteins bind to E1 during fusion.	bind
5758	1	2758	5	10	NULL	NULL	NULL	CSL	GP		bind		non specific;;dose-dependently			Caco-2 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_10_5282_s_234	10496907	(A) Dose-dependent binding of CSL to Caco-2 cells, corrected for nonspecific binding.	bind
8847	1	2758	7	10	NULL	NULL	NULL	CSL	GP		bind		non specific;;dose-dependently			Caco-2 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_10_5282_s_234	10496907	(A) Dose-dependent binding of CSL to Caco-2 cells, corrected for nonspecific binding.	bind
5760	1	2759	5	10	NULL	NULL	NULL	dTAFII110	GP		bind					NFATp	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_10_3503_s_171	11313476	(A) dTAFII110 binds to NFATp.	bind
8848	1	2759	7	10	NULL	NULL	NULL	dTAFII110	GP		bind					NFATp	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_10_3503_s_171	11313476	(A) dTAFII110 binds to NFATp.	bind
5761	1	2760	5	10	NULL	NULL	NULL	DtxR	GP		bind					IRP6	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_17_4846_s_140	12169610	(A) DtxR binding of IRP6 requires a divalent transitional metal ion, such as Co2+.	bind
5762	2	2760	5	10	NULL	NULL	NULL	statement 1	Process		require					Co2+	Chemical	divalent transitional metal ion			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_17_4846_s_140	12169610	(A) DtxR binding of IRP6 requires a divalent transitional metal ion, such as Co2+.	bind
8849	1	2760	7	10	NULL	NULL	NULL	DtxR	GP		bind					IRP6	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_17_4846_s_140	12169610	(A) DtxR binding of IRP6 requires a divalent transitional metal ion, such as Co2+.	bind
8850	2	2760	7	10	NULL	NULL	NULL	statement 1	Process		requires					Co2+	Chemical	divalent transitional metal ion			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_17_4846_s_140	12169610	(A) DtxR binding of IRP6 requires a divalent transitional metal ion, such as Co2+.	bind
5763	1	2761	5	10	NULL	NULL	NULL	Comm	GP		serves as					adaptor protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_36_1_5_s_54	12367500	(A) During a growth cone's approach to the midline, Comm serves as an adaptor protein binding to Robo as well as to Nedd4.	bind
5764	2	2761	5	10	NULL	NULL	NULL	Comm	GP		bind					Robo	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_36_1_5_s_54	12367500	(A) During a growth cone's approach to the midline, Comm serves as an adaptor protein binding to Robo as well as to Nedd4.	bind
5765	3	2761	5	10	NULL	NULL	NULL	Comm	GP		bind					Nedd4	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_36_1_5_s_54	12367500	(A) During a growth cone's approach to the midline, Comm serves as an adaptor protein binding to Robo as well as to Nedd4.	bind
5766	4	2761	5	10	NULL	NULL	NULL	statement 2	Process		occurs during					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_36_1_5_s_54	12367500	(A) During a growth cone's approach to the midline, Comm serves as an adaptor protein binding to Robo as well as to Nedd4.	bind
5767	5	2761	5	10	NULL	NULL	NULL	statement 3	Process		occurs during					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_36_1_5_s_54	12367500	(A) During a growth cone's approach to the midline, Comm serves as an adaptor protein binding to Robo as well as to Nedd4.	bind
46401	6	2761	5	10	NULL	NULL	NULL	growth cone	CellComponent		approach to					midline	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_neuron_36_1_5_s_54	12367500	(A) During a growth cone's approach to the midline, Comm serves as an adaptor protein binding to Robo as well as to Nedd4.	bind
8855	1	2761	7	10	NULL	NULL	NULL	Comm	GP		bind					Robo	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_36_1_5_s_54	12367500	(A) During a growth cone's approach to the midline, Comm serves as an adaptor protein binding to Robo as well as to Nedd4.	bind
8856	2	2761	7	10	NULL	NULL	NULL	Comm	GP		bind					Nedd4	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_36_1_5_s_54	12367500	(A) During a growth cone's approach to the midline, Comm serves as an adaptor protein binding to Robo as well as to Nedd4.	bind
8857	3	2761	7	10	NULL	NULL	NULL	Comm	GP		serves as an					adaptor protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_36_1_5_s_54	12367500	(A) During a growth cone's approach to the midline, Comm serves as an adaptor protein binding to Robo as well as to Nedd4.	bind
11754	4	2761	7	10	NULL	NULL	NULL	statement 1	Process		occur during					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_36_1_5_s_54	12367500	(A) During a growth cone's approach to the midline, Comm serves as an adaptor protein binding to Robo as well as to Nedd4.	bind
11755	5	2761	7	10	NULL	NULL	NULL	statement 3	Process		occur during					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_36_1_5_s_54	12367500	(A) During a growth cone's approach to the midline, Comm serves as an adaptor protein binding to Robo as well as to Nedd4.	bind
46402	6	2761	7	10	NULL	NULL	NULL	growth cone	CellComponent		approach to					midline	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_neuron_36_1_5_s_54	12367500	(A) During a growth cone's approach to the midline, Comm serves as an adaptor protein binding to Robo as well as to Nedd4.	bind
5768	2	2762	5	10	NULL	NULL	NULL	INS	GP	unidentified	bind					DAF-2 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_2_1_9_s_65	11782310	(A) During favorable growth conditions,  unc-64 and  unc-31 function to promote an as yet unidentified insulin-like ligand (INS) that binds to the DAF-2 receptor.	bind
5769	3	2762	5	10	NULL	NULL	NULL	unc-64	GP		promote					INS	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_2_1_9_s_65	11782310	(A) During favorable growth conditions,  unc-64 and  unc-31 function to promote an as yet unidentified insulin-like ligand (INS) that binds to the DAF-2 receptor.	bind
5770	4	2762	5	10	NULL	NULL	NULL	unc-31	GP		promote					INS	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_2_1_9_s_65	11782310	(A) During favorable growth conditions,  unc-64 and  unc-31 function to promote an as yet unidentified insulin-like ligand (INS) that binds to the DAF-2 receptor.	bind
5771	5	2762	5	10	NULL	NULL	NULL	statement 3	Process		occurs during					favorable growth conditions	Process				NULL		NULL	NULL	NULL	NULL	gw60_devcell_2_1_9_s_65	11782310	(A) During favorable growth conditions,  unc-64 and  unc-31 function to promote an as yet unidentified insulin-like ligand (INS) that binds to the DAF-2 receptor.	bind
5772	6	2762	5	10	NULL	NULL	NULL	statement 4	Process		occurs during					favorable growth conditions	Process				NULL		NULL	NULL	NULL	NULL	gw60_devcell_2_1_9_s_65	11782310	(A) During favorable growth conditions,  unc-64 and  unc-31 function to promote an as yet unidentified insulin-like ligand (INS) that binds to the DAF-2 receptor.	bind
11930	1	2762	5	10	NULL	NULL	NULL	insulin-like ligand	GP		is					INS	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_2_1_9_s_65	11782310	(A) During favorable growth conditions,  unc-64 and  unc-31 function to promote an as yet unidentified insulin-like ligand (INS) that binds to the DAF-2 receptor.	bind
8858	1	2762	7	10	NULL	NULL	NULL	insulin-like ligand	GP		bind					DAF-2 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_2_1_9_s_65	11782310	(A) During favorable growth conditions,  unc-64 and  unc-31 function to promote an as yet unidentified insulin-like ligand (INS) that binds to the DAF-2 receptor.	bind
8859	2	2762	7	10	NULL	NULL	NULL	insulin-like ligand	GP		is					INS	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_2_1_9_s_65	11782310	(A) During favorable growth conditions,  unc-64 and  unc-31 function to promote an as yet unidentified insulin-like ligand (INS) that binds to the DAF-2 receptor.	bind
8860	3	2762	7	10	NULL	NULL	NULL	 unc-64	GP		promote					INS	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_2_1_9_s_65	11782310	(A) During favorable growth conditions,  unc-64 and  unc-31 function to promote an as yet unidentified insulin-like ligand (INS) that binds to the DAF-2 receptor.	bind
8861	4	2762	7	10	NULL	NULL	NULL	unc-31	GP		promote					INS	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_2_1_9_s_65	11782310	(A) During favorable growth conditions,  unc-64 and  unc-31 function to promote an as yet unidentified insulin-like ligand (INS) that binds to the DAF-2 receptor.	bind
11756	5	2762	7	10	NULL	NULL	NULL	statement 3	Process		occur during					growth favourable condition	Process				NULL		NULL	NULL	NULL	NULL	gw60_devcell_2_1_9_s_65	11782310	(A) During favorable growth conditions,  unc-64 and  unc-31 function to promote an as yet unidentified insulin-like ligand (INS) that binds to the DAF-2 receptor.	bind
11757	6	2762	7	10	NULL	NULL	NULL	statement 4	Process		occur during					growth favourable condition	Process				NULL		NULL	NULL	NULL	NULL	gw60_devcell_2_1_9_s_65	11782310	(A) During favorable growth conditions,  unc-64 and  unc-31 function to promote an as yet unidentified insulin-like ligand (INS) that binds to the DAF-2 receptor.	bind
5773	1	2764	5	10	NULL	NULL	NULL	E2F	GP		bind					MCM4	GP			promoter	NULL	in serum-stimulated T98G cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_10_4546_s_84	15121871	(A) E2F binding  to the MCM4 promoter in serum-stimulated T98G cells as determined by ChIP (% total)  overlapped with the percentage of cells in S phase as determined by BrdU incorporation  and fluorescence-activated cell sorting.	bind
8862	1	2764	7	10	NULL	NULL	NULL	E2F	GP		bind					MCM4	GP			promoter	NULL	serum-stimulated T98G cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_10_4546_s_84	15121871	(A) E2F binding  to the MCM4 promoter in serum-stimulated T98G cells as determined by ChIP (% total)  overlapped with the percentage of cells in S phase as determined by BrdU incorporation  and fluorescence-activated cell sorting.	bind
5774	1	2765	5	10	NULL	NULL	NULL	AFP	GP	native	bind					MDM	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_3_507_s_101	12176010	(A) Effect of anti-AFP antibodies (anti-AFP) or its isotype on the binding of native [125]AFP to MDM.	bind
8863	1	2765	7	10	NULL	NULL	NULL	[125]AFP	GP	native	bind					MDM	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_3_507_s_101	12176010	(A) Effect of anti-AFP antibodies (anti-AFP) or its isotype on the binding of native [125]AFP to MDM.	bind
5788	1	2766	5	10	NULL	NULL	NULL	NF-kappaB	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_1_206_s_136	9864217	(A) Effect of CHX on induction of the DNA binding of NF-kappaB by LPS with or without pretreatment with IFN-gamma.	bind
5789	2	2766	5	10	NULL	NULL	NULL	LPS	Chemical		induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_1_206_s_136	9864217	(A) Effect of CHX on induction of the DNA binding of NF-kappaB by LPS with or without pretreatment with IFN-gamma.	bind
8864	1	2766	7	10	NULL	NULL	NULL	NF-kappaB	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_1_206_s_136	9864217	(A) Effect of CHX on induction of the DNA binding of NF-kappaB by LPS with or without pretreatment with IFN-gamma.	bind
9483	2	2766	7	10	NULL	NULL	NULL	LPS	Chemical		induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_1_206_s_136	9864217	(A) Effect of CHX on induction of the DNA binding of NF-kappaB by LPS with or without pretreatment with IFN-gamma.	bind
5793	1	2767	5	10	NULL	NULL	NULL	HEK 293 cells	Cell		express		stably			AT1R - YFP	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_8_1495_s_178	12721105	(a) Effect of PMA on [3]AII binding to HEK 293 cells stably expressing AT1R - YFP. Results are expressed as percent of the maximal specific binding recorded in the control curve (8 nM of radioligand).	bind
5794	2	2767	5	10	NULL	NULL	NULL	AII	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_8_1495_s_178	12721105	(a) Effect of PMA on [3]AII binding to HEK 293 cells stably expressing AT1R - YFP. Results are expressed as percent of the maximal specific binding recorded in the control curve (8 nM of radioligand).	bind
8874	1	2767	7	10	NULL	NULL	NULL	HEK 293 cells	Cell		express					AT1R - YFP	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_8_1495_s_178	12721105	(a) Effect of PMA on [3]AII binding to HEK 293 cells stably expressing AT1R - YFP. Results are expressed as percent of the maximal specific binding recorded in the control curve (8 nM of radioligand).	bind
46404	2	2767	7	10	NULL	NULL	NULL	AII	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_8_1495_s_178	12721105	(a) Effect of PMA on [3]AII binding to HEK 293 cells stably expressing AT1R - YFP. Results are expressed as percent of the maximal specific binding recorded in the control curve (8 nM of radioligand).	bind
5795	1	2768	5	10	NULL	NULL	NULL	p97	GP		bind					RanBP2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_8_12_2379_s_190	9398662	(A) Effect of Ran on the binding of p97 to RanBP2.	bind
8875	1	2768	7	10	NULL	NULL	NULL	p97	GP		bind					RanBP2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_8_12_2379_s_190	9398662	(A) Effect of Ran on the binding of p97 to RanBP2.	bind
5796	1	2769	5	10	NULL	NULL	NULL	Bas1p	GP		bind					ADE5,7	GP			promoter	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_23_7901_s_326	11689683	(A) Effect of SAICAR and AICAR on cooperative in vitro binding of Bas1p and Bas2p to the  ADE5,7 promoter.	bind
5797	2	2769	5	10	NULL	NULL	NULL	Bas2p	GP		bind					ADE5,7	GP			promoter	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_23_7901_s_326	11689683	(A) Effect of SAICAR and AICAR on cooperative in vitro binding of Bas1p and Bas2p to the  ADE5,7 promoter.	bind
5798	3	2769	5	10	NULL	NULL	NULL	statement 1	Process		occurs in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_23_7901_s_326	11689683	(A) Effect of SAICAR and AICAR on cooperative in vitro binding of Bas1p and Bas2p to the  ADE5,7 promoter.	bind
8876	1	2769	7	10	NULL	NULL	NULL	Bas1p	GP		bind					ADE5,7	GP			promoter	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_23_7901_s_326	11689683	(A) Effect of SAICAR and AICAR on cooperative in vitro binding of Bas1p and Bas2p to the  ADE5,7 promoter.	bind
8877	2	2769	7	10	NULL	NULL	NULL	Bas2p	GP		bind					ADE5,7	GP			promoter	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_23_7901_s_326	11689683	(A) Effect of SAICAR and AICAR on cooperative in vitro binding of Bas1p and Bas2p to the  ADE5,7 promoter.	bind
8894	3	2769	7	10	NULL	NULL	NULL	statement 1	Process		occurs in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_23_7901_s_326	11689683	(A) Effect of SAICAR and AICAR on cooperative in vitro binding of Bas1p and Bas2p to the  ADE5,7 promoter.	bind
5799	1	2770	5	10	NULL	NULL	NULL	SIL	CellComponent		bind					KG-1a	Cell				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1509_1_299_s_218	11118541	(A) Effect of the lipid concentration on the degree of SIL binding to KG-1a.	bind
8900	1	2770	7	10	NULL	NULL	NULL	SIL	CellComponent		bind					KG-1a	Cell				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1509_1_299_s_218	11118541	(A) Effect of the lipid concentration on the degree of SIL binding to KG-1a.	bind
5801	1	2773	5	10	NULL	NULL	NULL	arsenite	Chemical		induce					ERK	GP	activation			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5178_s_226	9710602	(A) Effects of suramin and tyrphostin AG1478 on arsenite-induced ERK activation.	bind
8981	1	2773	7	10	NULL	NULL	NULL	arsenite	Chemical		induce					ERK	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5178_s_226	9710602	(A) Effects of suramin and tyrphostin AG1478 on arsenite-induced ERK activation.	bind
5802	1	2774	5	10	NULL	NULL	NULL	HEXIM1	GP	isolated	bind			NLS		7SK	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_12_5094_s_146	15169877	(A) Efficient in vivo binding of the isolated NLS of HEXIM1  to 7SK but not P-TEFb.	bind
5803	2	2774	5	10	NULL	NULL	NULL	HEXIM1	GP	isolated	does not bind			NLS		P-TEFb	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_12_5094_s_146	15169877	(A) Efficient in vivo binding of the isolated NLS of HEXIM1  to 7SK but not P-TEFb.	bind
8982	1	2774	7	10	NULL	NULL	NULL	HEXIM1	GP	isolated	bind			NLS		7SK	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_12_5094_s_146	15169877	(A) Efficient in vivo binding of the isolated NLS of HEXIM1  to 7SK but not P-TEFb.	bind
8983	2	2774	7	10	NULL	NULL	NULL	HEXIM1	GP	isolated	does not bind			NLS		P-TEFb	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_12_5094_s_146	15169877	(A) Efficient in vivo binding of the isolated NLS of HEXIM1  to 7SK but not P-TEFb.	bind
5804	1	2775	5	10	NULL	NULL	NULL	EKLF	GP		bind					beta gene	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_102_s_238	9418858	(A) EKLF bound to the beta gene recruits a subcomplex of the transcriptional machinery and enables formation of a transcription initiation complex (IC) of the beta gene together with TFIID containing TATA box-binding protein (TBP), RNA polymerase II (pol II) holoenzyme, and probably other subcomplexes recruited by other transcriptional activators.	bind
5805	2	2775	5	10	NULL	NULL	NULL	statement 1	Process		recruit					transcriptional machinery	GP	a subcomplex of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_102_s_238	9418858	(A) EKLF bound to the beta gene recruits a subcomplex of the transcriptional machinery and enables formation of a transcription initiation complex (IC) of the beta gene together with TFIID containing TATA box-binding protein (TBP), RNA polymerase II (pol II) holoenzyme, and probably other subcomplexes recruited by other transcriptional activators.	bind
5806	3	2775	5	10	NULL	NULL	NULL	statement 1	Process		enables					IC of beta gene	GP	formation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_102_s_238	9418858	(A) EKLF bound to the beta gene recruits a subcomplex of the transcriptional machinery and enables formation of a transcription initiation complex (IC) of the beta gene together with TFIID containing TATA box-binding protein (TBP), RNA polymerase II (pol II) holoenzyme, and probably other subcomplexes recruited by other transcriptional activators.	bind
5807	4	2775	5	10	NULL	NULL	NULL	IC	GP		is					transcription initiation complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_102_s_238	9418858	(A) EKLF bound to the beta gene recruits a subcomplex of the transcriptional machinery and enables formation of a transcription initiation complex (IC) of the beta gene together with TFIID containing TATA box-binding protein (TBP), RNA polymerase II (pol II) holoenzyme, and probably other subcomplexes recruited by other transcriptional activators.	bind
5808	5	2775	5	10	NULL	NULL	NULL	statement 3	Process		occurs along with					TBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_102_s_238	9418858	(A) EKLF bound to the beta gene recruits a subcomplex of the transcriptional machinery and enables formation of a transcription initiation complex (IC) of the beta gene together with TFIID containing TATA box-binding protein (TBP), RNA polymerase II (pol II) holoenzyme, and probably other subcomplexes recruited by other transcriptional activators.	bind
5809	6	2775	5	10	NULL	NULL	NULL	TBP	GP		is					TATA box-binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_102_s_238	9418858	(A) EKLF bound to the beta gene recruits a subcomplex of the transcriptional machinery and enables formation of a transcription initiation complex (IC) of the beta gene together with TFIID containing TATA box-binding protein (TBP), RNA polymerase II (pol II) holoenzyme, and probably other subcomplexes recruited by other transcriptional activators.	bind
5810	7	2775	5	10	NULL	NULL	NULL	statement 3	Process		occurs along with					pol II	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_102_s_238	9418858	(A) EKLF bound to the beta gene recruits a subcomplex of the transcriptional machinery and enables formation of a transcription initiation complex (IC) of the beta gene together with TFIID containing TATA box-binding protein (TBP), RNA polymerase II (pol II) holoenzyme, and probably other subcomplexes recruited by other transcriptional activators.	bind
5811	8	2775	5	10	NULL	NULL	NULL	pol II	GP		is					RNA polymerase II holoenzyme	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_102_s_238	9418858	(A) EKLF bound to the beta gene recruits a subcomplex of the transcriptional machinery and enables formation of a transcription initiation complex (IC) of the beta gene together with TFIID containing TATA box-binding protein (TBP), RNA polymerase II (pol II) holoenzyme, and probably other subcomplexes recruited by other transcriptional activators.	bind
5812	9	2775	5	10	NULL	NULL	NULL	transcriptional activators	GP		recruit					subcomplexes	GP	other			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_102_s_238	9418858	(A) EKLF bound to the beta gene recruits a subcomplex of the transcriptional machinery and enables formation of a transcription initiation complex (IC) of the beta gene together with TFIID containing TATA box-binding protein (TBP), RNA polymerase II (pol II) holoenzyme, and probably other subcomplexes recruited by other transcriptional activators.	bind
5813	10	2775	5	10	NULL	NULL	NULL	statement 3	Process		occurs along with		probably			statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_102_s_238	9418858	(A) EKLF bound to the beta gene recruits a subcomplex of the transcriptional machinery and enables formation of a transcription initiation complex (IC) of the beta gene together with TFIID containing TATA box-binding protein (TBP), RNA polymerase II (pol II) holoenzyme, and probably other subcomplexes recruited by other transcriptional activators.	bind
8984	1	2775	7	10	NULL	NULL	NULL	EKLF	GP		bind					beta gene	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_102_s_238	9418858	(A) EKLF bound to the beta gene recruits a subcomplex of the transcriptional machinery and enables formation of a transcription initiation complex (IC) of the beta gene together with TFIID containing TATA box-binding protein (TBP), RNA polymerase II (pol II) holoenzyme, and probably other subcomplexes recruited by other transcriptional activators.	bind
8985	2	2775	7	10	NULL	NULL	NULL	statement 1	Process		recruits					transcriptional machinery	GP	subcomplex of the			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_102_s_238	9418858	(A) EKLF bound to the beta gene recruits a subcomplex of the transcriptional machinery and enables formation of a transcription initiation complex (IC) of the beta gene together with TFIID containing TATA box-binding protein (TBP), RNA polymerase II (pol II) holoenzyme, and probably other subcomplexes recruited by other transcriptional activators.	bind
8986	3	2775	7	10	NULL	NULL	NULL	statement 2	Process		enables 					IC of beta gene	GP	formation of 			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_102_s_238	9418858	(A) EKLF bound to the beta gene recruits a subcomplex of the transcriptional machinery and enables formation of a transcription initiation complex (IC) of the beta gene together with TFIID containing TATA box-binding protein (TBP), RNA polymerase II (pol II) holoenzyme, and probably other subcomplexes recruited by other transcriptional activators.	bind
8990	4	2775	7	10	NULL	NULL	NULL	transcription initiation complex	GP		consist of					TFIID containing TATA box-binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_102_s_238	9418858	(A) EKLF bound to the beta gene recruits a subcomplex of the transcriptional machinery and enables formation of a transcription initiation complex (IC) of the beta gene together with TFIID containing TATA box-binding protein (TBP), RNA polymerase II (pol II) holoenzyme, and probably other subcomplexes recruited by other transcriptional activators.	bind
8991	5	2775	7	10	NULL	NULL	NULL	transcription initiation complex	GP		consist of					RNA polymerase II holoenzyme	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_102_s_238	9418858	(A) EKLF bound to the beta gene recruits a subcomplex of the transcriptional machinery and enables formation of a transcription initiation complex (IC) of the beta gene together with TFIID containing TATA box-binding protein (TBP), RNA polymerase II (pol II) holoenzyme, and probably other subcomplexes recruited by other transcriptional activators.	bind
8992	6	2775	7	10	NULL	NULL	NULL	transcription initiation complex	GP		consist of					 transcriptional activators	GP	subcomplexes recruited by other			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_102_s_238	9418858	(A) EKLF bound to the beta gene recruits a subcomplex of the transcriptional machinery and enables formation of a transcription initiation complex (IC) of the beta gene together with TFIID containing TATA box-binding protein (TBP), RNA polymerase II (pol II) holoenzyme, and probably other subcomplexes recruited by other transcriptional activators.	bind
8993	7	2775	7	10	NULL	NULL	NULL	IC	GP		is					transcription initiation complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_102_s_238	9418858	(A) EKLF bound to the beta gene recruits a subcomplex of the transcriptional machinery and enables formation of a transcription initiation complex (IC) of the beta gene together with TFIID containing TATA box-binding protein (TBP), RNA polymerase II (pol II) holoenzyme, and probably other subcomplexes recruited by other transcriptional activators.	bind
8994	8	2775	7	10	NULL	NULL	NULL	TBP	GP		is					TATA box-binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_102_s_238	9418858	(A) EKLF bound to the beta gene recruits a subcomplex of the transcriptional machinery and enables formation of a transcription initiation complex (IC) of the beta gene together with TFIID containing TATA box-binding protein (TBP), RNA polymerase II (pol II) holoenzyme, and probably other subcomplexes recruited by other transcriptional activators.	bind
8995	9	2775	7	10	NULL	NULL	NULL	pol II	GP		is					RNA polymerase II holoenzyme	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_102_s_238	9418858	(A) EKLF bound to the beta gene recruits a subcomplex of the transcriptional machinery and enables formation of a transcription initiation complex (IC) of the beta gene together with TFIID containing TATA box-binding protein (TBP), RNA polymerase II (pol II) holoenzyme, and probably other subcomplexes recruited by other transcriptional activators.	bind
5814	1	2776	5	10	NULL	NULL	NULL	Isw2 complex	GP		bind					NCPs	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_21_9165_s_172	16227570	(A) Electromobility  shift assay measuring binding of Isw2 complex to wild-type or mutant NCPs. NCPs bound  by Isw2 complex and unbound NCPs are indicated by white and black arrows, respectively.	bind
5815	2	2776	5	10	NULL	NULL	NULL	Isw2 complex	GP		bind					NCPs	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_21_9165_s_172	16227570	(A) Electromobility  shift assay measuring binding of Isw2 complex to wild-type or mutant NCPs. NCPs bound  by Isw2 complex and unbound NCPs are indicated by white and black arrows, respectively.	bind
8987	1	2776	7	10	NULL	NULL	NULL	Isw2 complex	GP		bind					NCPs	GP	wild-type			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_21_9165_s_172	16227570	(A) Electromobility  shift assay measuring binding of Isw2 complex to wild-type or mutant NCPs. NCPs bound  by Isw2 complex and unbound NCPs are indicated by white and black arrows, respectively.	bind
8988	2	2776	7	10	NULL	NULL	NULL	Isw2 complex	GP		bind					NCPs	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_21_9165_s_172	16227570	(A) Electromobility  shift assay measuring binding of Isw2 complex to wild-type or mutant NCPs. NCPs bound  by Isw2 complex and unbound NCPs are indicated by white and black arrows, respectively.	bind
5816	1	2777	5	10	NULL	NULL	NULL	TBP molecules	GP	full-length;;wild-type	bind					U6	GP	human		promoter	NULL		NULL	NULL	NULL	NULL	gw60_cell_108_5_615_s_28	11893333	(A) Electrophoretic mobility retardation analysis of full-length wild-type and mutant TBP molecules binding to the human U6 promoter.	bind
5817	2	2777	5	10	NULL	NULL	NULL	TBP molecules	GP	mutant	bind					U6	GP	human		promoter	NULL		NULL	NULL	NULL	NULL	gw60_cell_108_5_615_s_28	11893333	(A) Electrophoretic mobility retardation analysis of full-length wild-type and mutant TBP molecules binding to the human U6 promoter.	bind
8865	1	2777	7	10	NULL	NULL	NULL	TBP	GP	 full-length;;wild-type	bind					U6	GP	human		promoter	NULL		NULL	NULL	NULL	NULL	gw60_cell_108_5_615_s_28	11893333	(A) Electrophoretic mobility retardation analysis of full-length wild-type and mutant TBP molecules binding to the human U6 promoter.	bind
8866	2	2777	7	10	NULL	NULL	NULL	TBP	GP	mutant	bind					U6	GP	human		promoter	NULL		NULL	NULL	NULL	NULL	gw60_cell_108_5_615_s_28	11893333	(A) Electrophoretic mobility retardation analysis of full-length wild-type and mutant TBP molecules binding to the human U6 promoter.	bind
5818	1	2780	5	10	NULL	NULL	NULL	IgM antibodies	GP		bind					LDL	GP	oxidized			NULL	sera of apoE-deficient mice	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_734_s_176	10073981	(A) ELISA assay showing the binding of IgM and IgG antibodies to oxidized LDL in the sera of apoE-deficient mice.	bind
5819	2	2780	5	10	NULL	NULL	NULL	IgG antibodies	GP		bind					LDL	GP	oxidized			NULL	sera of apoE-deficient mice	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_734_s_176	10073981	(A) ELISA assay showing the binding of IgM and IgG antibodies to oxidized LDL in the sera of apoE-deficient mice.	bind
8867	1	2780	7	10	NULL	NULL	NULL	IgM antibodies	GP		bind					LDL	GP	oxidized			NULL	in the sera of apoE-deficient mice	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_734_s_176	10073981	(A) ELISA assay showing the binding of IgM and IgG antibodies to oxidized LDL in the sera of apoE-deficient mice.	bind
8868	2	2780	7	10	NULL	NULL	NULL	IgG antibodies	GP		bind					LDL	GP	oxidized			NULL	in the sera of apoE-deficient mice	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_734_s_176	10073981	(A) ELISA assay showing the binding of IgM and IgG antibodies to oxidized LDL in the sera of apoE-deficient mice.	bind
5820	1	2781	5	10	NULL	NULL	NULL	ELMO1-GFP	GP		bind					Dock180	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_1_27_s_230	11595183	(A) ELMO1-GFP binds Dock180.	bind
8869	1	2781	7	10	NULL	NULL	NULL	ELMO1-GFP	GP		bind					Dock180	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_1_27_s_230	11595183	(A) ELMO1-GFP binds Dock180.	bind
5822	1	2784	5	10	NULL	NULL	NULL	YY1	GP		bind					b4C	GP	wt			NULL		NULL	NULL	NULL	NULL	gw60_development_129_16_3887_s_220	12135926	(A) EMSA competition experiments showing the ability of specific mutations to interfere with the binding of YY1 and NF-Y to b4Cwt.	bind
5823	2	2784	5	10	NULL	NULL	NULL	NF-Y	GP		bind					b4C	GP	wt			NULL		NULL	NULL	NULL	NULL	gw60_development_129_16_3887_s_220	12135926	(A) EMSA competition experiments showing the ability of specific mutations to interfere with the binding of YY1 and NF-Y to b4Cwt.	bind
8870	1	2784	7	10	NULL	NULL	NULL	YY1	GP		bind					b4C	GP	wt			NULL		NULL	NULL	NULL	NULL	gw60_development_129_16_3887_s_220	12135926	(A) EMSA competition experiments showing the ability of specific mutations to interfere with the binding of YY1 and NF-Y to b4Cwt.	bind
8871	2	2784	7	10	NULL	NULL	NULL	NF-Y	GP		bind					b4C	GP	wt			NULL		NULL	NULL	NULL	NULL	gw60_development_129_16_3887_s_220	12135926	(A) EMSA competition experiments showing the ability of specific mutations to interfere with the binding of YY1 and NF-Y to b4Cwt.	bind
5826	1	2785	5	10	NULL	NULL	NULL	GST-CP2b	GP	recombinant	bind		weakly			probe DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_14_6005_s_250	15988015	(A) EMSA demonstrated that recombinant GST-CP2b bound very weakly to the probe DNA,  while other isoforms showed strong DNA binding activities (a).	bind
8873	1	2785	7	10	NULL	NULL	NULL	GST-CP2b	GP	recombinant	bind		very weakly			probe DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_14_6005_s_250	15988015	(A) EMSA demonstrated that recombinant GST-CP2b bound very weakly to the probe DNA,  while other isoforms showed strong DNA binding activities (a).	bind
5828	1	2786	5	10	NULL	NULL	NULL	AP-1	GP		bind					fra-1 oligonucleotide	NucleicAcid			TRE	NULL	FRTL-5MEK	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_12_4401_s_250	12773579	(A) EMSA of AP-1 binding to the  fra-1 TRE oligonucleotide in the FRTL-5-derived cell clones expressing the constitutively  active form of MEK and/or Rac (FRTL-5MEK, FRTL-5Rac, and FRTL-5MEK/Rac).	bind
5829	2	2786	5	10	NULL	NULL	NULL	FRTL-5-derived cell clones	Cell		express					MEK	GP	constitutively active form of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_12_4401_s_250	12773579	(A) EMSA of AP-1 binding to the  fra-1 TRE oligonucleotide in the FRTL-5-derived cell clones expressing the constitutively  active form of MEK and/or Rac (FRTL-5MEK, FRTL-5Rac, and FRTL-5MEK/Rac).	bind
5830	3	2786	5	10	NULL	NULL	NULL	FRTL-5MEK	Cell		is					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_12_4401_s_250	12773579	(A) EMSA of AP-1 binding to the  fra-1 TRE oligonucleotide in the FRTL-5-derived cell clones expressing the constitutively  active form of MEK and/or Rac (FRTL-5MEK, FRTL-5Rac, and FRTL-5MEK/Rac).	bind
5831	4	2786	5	10	NULL	NULL	NULL	FRTL-5-derived cell clones	Cell		express					Rac	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_12_4401_s_250	12773579	(A) EMSA of AP-1 binding to the  fra-1 TRE oligonucleotide in the FRTL-5-derived cell clones expressing the constitutively  active form of MEK and/or Rac (FRTL-5MEK, FRTL-5Rac, and FRTL-5MEK/Rac).	bind
5832	5	2786	5	10	NULL	NULL	NULL	FRTL-5Rac	Cell		is					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_12_4401_s_250	12773579	(A) EMSA of AP-1 binding to the  fra-1 TRE oligonucleotide in the FRTL-5-derived cell clones expressing the constitutively  active form of MEK and/or Rac (FRTL-5MEK, FRTL-5Rac, and FRTL-5MEK/Rac).	bind
5833	6	2786	5	10	NULL	NULL	NULL	statement 2	Process		occurs simultaneously with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_12_4401_s_250	12773579	(A) EMSA of AP-1 binding to the  fra-1 TRE oligonucleotide in the FRTL-5-derived cell clones expressing the constitutively  active form of MEK and/or Rac (FRTL-5MEK, FRTL-5Rac, and FRTL-5MEK/Rac).	bind
5834	7	2786	5	10	NULL	NULL	NULL	statement 6	Process		is					FRTL-5MEK/Rac	Cell				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_12_4401_s_250	12773579	(A) EMSA of AP-1 binding to the  fra-1 TRE oligonucleotide in the FRTL-5-derived cell clones expressing the constitutively  active form of MEK and/or Rac (FRTL-5MEK, FRTL-5Rac, and FRTL-5MEK/Rac).	bind
5835	8	2786	5	10	NULL	NULL	NULL	AP-1	GP		bind					fra-1 TRE oligonucleotide	NucleicAcid				NULL	FRTL-5Rac	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_12_4401_s_250	12773579	(A) EMSA of AP-1 binding to the  fra-1 TRE oligonucleotide in the FRTL-5-derived cell clones expressing the constitutively  active form of MEK and/or Rac (FRTL-5MEK, FRTL-5Rac, and FRTL-5MEK/Rac).	bind
5836	9	2786	5	10	NULL	NULL	NULL	AP-1	GP		bind					fra-1 TRE oligonucleotide	NucleicAcid				NULL	FRTL-5MEK/Rac	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_12_4401_s_250	12773579	(A) EMSA of AP-1 binding to the  fra-1 TRE oligonucleotide in the FRTL-5-derived cell clones expressing the constitutively  active form of MEK and/or Rac (FRTL-5MEK, FRTL-5Rac, and FRTL-5MEK/Rac).	bind
8996	1	2786	7	10	NULL	0	NULL	 AP-1			bind					 fra-1oligonucleotide				TRE 	NULL	FRTL-5MEK	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_12_4401_s_250	12773579	(A) EMSA of AP-1 binding to the  fra-1 TRE oligonucleotide in the FRTL-5-derived cell clones expressing the constitutively  active form of MEK and/or Rac (FRTL-5MEK, FRTL-5Rac, and FRTL-5MEK/Rac).	bind
8997	2	2786	7	10	NULL	NULL	NULL	FRTL-5-derived cell	Cell		express					MEK	GP	constitutively active form of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_12_4401_s_250	12773579	(A) EMSA of AP-1 binding to the  fra-1 TRE oligonucleotide in the FRTL-5-derived cell clones expressing the constitutively  active form of MEK and/or Rac (FRTL-5MEK, FRTL-5Rac, and FRTL-5MEK/Rac).	bind
8998	3	2786	7	10	NULL	NULL	NULL	FRTL-5-derived cell	Cell		express					Rac	GP	constitutively active form of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_12_4401_s_250	12773579	(A) EMSA of AP-1 binding to the  fra-1 TRE oligonucleotide in the FRTL-5-derived cell clones expressing the constitutively  active form of MEK and/or Rac (FRTL-5MEK, FRTL-5Rac, and FRTL-5MEK/Rac).	bind
8999	4	2786	7	10	NULL	NULL	NULL	statement 2	Process		is					FRTL-5MEK	Cell				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_12_4401_s_250	12773579	(A) EMSA of AP-1 binding to the  fra-1 TRE oligonucleotide in the FRTL-5-derived cell clones expressing the constitutively  active form of MEK and/or Rac (FRTL-5MEK, FRTL-5Rac, and FRTL-5MEK/Rac).	bind
9000	5	2786	7	10	NULL	NULL	NULL	statement 3	Process		is					FRTL-5Rac	Cell				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_12_4401_s_250	12773579	(A) EMSA of AP-1 binding to the  fra-1 TRE oligonucleotide in the FRTL-5-derived cell clones expressing the constitutively  active form of MEK and/or Rac (FRTL-5MEK, FRTL-5Rac, and FRTL-5MEK/Rac).	bind
9001	6	2786	7	10	NULL	NULL	NULL	FRTL-5-derived cell	Cell		express					MEK/Rac	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_12_4401_s_250	12773579	(A) EMSA of AP-1 binding to the  fra-1 TRE oligonucleotide in the FRTL-5-derived cell clones expressing the constitutively  active form of MEK and/or Rac (FRTL-5MEK, FRTL-5Rac, and FRTL-5MEK/Rac).	bind
11760	7	2786	7	10	NULL	NULL	NULL	statement 2 	Process		occur simultaneously with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_12_4401_s_250	12773579	(A) EMSA of AP-1 binding to the  fra-1 TRE oligonucleotide in the FRTL-5-derived cell clones expressing the constitutively  active form of MEK and/or Rac (FRTL-5MEK, FRTL-5Rac, and FRTL-5MEK/Rac).	bind
5837	1	2790	5	10	NULL	NULL	NULL	RBP-Jkappa proteins	GP	endogenous	bind		strongly			GST-SHARP	GP	immobilized	2002-3664		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10379_s_194	16287852	(A) Endogenous RBP-Jkappa proteins bind strongly to GST-SHARP(2002-3664) immobilized on glutathione Sepharose  beads.	bind
9002	1	2790	7	10	NULL	NULL	NULL	RBP-Jkappa proteins	GP	endogenous	bind		strongly			GST-SHARP	GP	immobilized	2002-3664		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10379_s_194	16287852	(A) Endogenous RBP-Jkappa proteins bind strongly to GST-SHARP(2002-3664) immobilized on glutathione Sepharose  beads.	bind
5838	1	2791	5	10	NULL	NULL	NULL	TRF2	GP	endogenous	bind					POT1	GP				NULL	IMR90 fibroblasts	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_3_1070_s_211	15657433	(A) Endogenous TRF2 bound to POT1 in IMR90 fibroblasts  by coimmunoprecipitation.	bind
9003	1	2791	7	10	NULL	NULL	NULL	TRF2	GP	endogenous	bind					 POT1	GP				NULL	IMR90 fibroblasts	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_3_1070_s_211	15657433	(A) Endogenous TRF2 bound to POT1 in IMR90 fibroblasts  by coimmunoprecipitation.	bind
5839	1	2792	5	10	NULL	NULL	NULL	Ent3p	GP		bind					clathrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_5_3_499_s_196	12967568	(A) Ent3p binds clathrin.	bind
9004	1	2792	7	10	NULL	NULL	NULL	Ent3p 	GP		bind					clathrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_5_3_499_s_196	12967568	(A) Ent3p binds clathrin.	bind
5840	1	2795	5	10	NULL	NULL	NULL	ERKs	GP		does not bind					Mxi2	GP	deletion mutant form lacking	C terminus		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_9_3079_s_293	12697810	(A) ERKs cannot bind  to a deletion mutant form of Mxi2 lacking the C terminus.	bind
9005	1	2795	7	10	NULL	NULL	NULL	ERKs	GP		does not bind					Mxi2 	GP	deletion mutant form lacking	C terminus		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_9_3079_s_293	12697810	(A) ERKs cannot bind  to a deletion mutant form of Mxi2 lacking the C terminus.	bind
5841	1	2797	5	10	NULL	NULL	NULL	ETO	GP		bind					HDAC-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6470_s_167	11533236	(A) ETO binds HDAC-1, HDAC-2, and HDAC-3.	bind
5842	2	2797	5	10	NULL	NULL	NULL	ETO	GP		bind					HDAC-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6470_s_167	11533236	(A) ETO binds HDAC-1, HDAC-2, and HDAC-3.	bind
5843	3	2797	5	10	NULL	NULL	NULL	ETO	GP		bind					HDAC-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6470_s_167	11533236	(A) ETO binds HDAC-1, HDAC-2, and HDAC-3.	bind
9006	1	2797	7	10	NULL	NULL	NULL	ETO	GP		binds					HDAC-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6470_s_167	11533236	(A) ETO binds HDAC-1, HDAC-2, and HDAC-3.	bind
9007	2	2797	7	10	NULL	NULL	NULL	ETO	GP		bind					HDAC-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6470_s_167	11533236	(A) ETO binds HDAC-1, HDAC-2, and HDAC-3.	bind
9008	3	2797	7	10	NULL	NULL	NULL	ETO	GP		bind					HDAC-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6470_s_167	11533236	(A) ETO binds HDAC-1, HDAC-2, and HDAC-3.	bind
5844	1	2798	5	10	NULL	NULL	NULL	peptide	AminoAcid		bind					deltaSET7/9 	GP		E-330 A		NULL		NULL	NULL	NULL	NULL	gw60_cell_111_1_105_s_216	12372304	(A) Example of ITC trace (upper) and fitted binding curve (lower) of peptide binding to deltaSET7/9 E-330 A.  (B) Summary of dissociation constants for peptide and AdoMet binding to SET7/9 constructs monitored by ITC and fluorescence spectroscopy.	bind
5845	2	2798	5	10	NULL	NULL	NULL	AdoMet	GP		bind					SET7/9 constructs	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_111_1_105_s_216	12372304	(A) Example of ITC trace (upper) and fitted binding curve (lower) of peptide binding to deltaSET7/9 E-330 A.  (B) Summary of dissociation constants for peptide and AdoMet binding to SET7/9 constructs monitored by ITC and fluorescence spectroscopy.	bind
9009	1	2798	7	10	NULL	NULL	NULL	peptide	AminoAcid		bind					deltaSET7/9	GP		E-330 A		NULL		NULL	NULL	NULL	NULL	gw60_cell_111_1_105_s_216	12372304	(A) Example of ITC trace (upper) and fitted binding curve (lower) of peptide binding to deltaSET7/9 E-330 A.  (B) Summary of dissociation constants for peptide and AdoMet binding to SET7/9 constructs monitored by ITC and fluorescence spectroscopy.	bind
9010	2	2798	7	10	NULL	NULL	NULL	AdoMet	GP		bind					SET7/9 constructs	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_111_1_105_s_216	12372304	(A) Example of ITC trace (upper) and fitted binding curve (lower) of peptide binding to deltaSET7/9 E-330 A.  (B) Summary of dissociation constants for peptide and AdoMet binding to SET7/9 constructs monitored by ITC and fluorescence spectroscopy.	bind
5847	1	2799	5	10	NULL	NULL	NULL	IBB	AminoAcid		is					importin beta binding fragment of importin	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_104_1_83_s_82	11163242	(A) Excess of NLS peptide  and of the importin beta binding fragment of importin   (IBB) promotes microtubule  assembly in  Xenopus M phase extracts.	bind
5848	2	2799	5	10	NULL	NULL	NULL	NLS peptide	AminoAcid	excess	promote					microtubule assembly	Process				NULL	in Xenopus M phase extracts	NULL	NULL	NULL	NULL	gw60_cell_104_1_83_s_82	11163242	(A) Excess of NLS peptide  and of the importin beta binding fragment of importin   (IBB) promotes microtubule  assembly in  Xenopus M phase extracts.	bind
5849	3	2799	5	10	NULL	NULL	NULL	IBB	GP	excess of 	promote					microtubule assembly	Process				NULL	in Xenopus M phase extracts	NULL	NULL	NULL	NULL	gw60_cell_104_1_83_s_82	11163242	(A) Excess of NLS peptide  and of the importin beta binding fragment of importin   (IBB) promotes microtubule  assembly in  Xenopus M phase extracts.	bind
9011	1	2799	7	10	NULL	NULL	NULL	NLS peptide	AminoAcid	excess of	promotes					microtubule assembly	Process				NULL	Xenopus M phase extracts	NULL	NULL	NULL	NULL	gw60_cell_104_1_83_s_82	11163242	(A) Excess of NLS peptide  and of the importin beta binding fragment of importin   (IBB) promotes microtubule  assembly in  Xenopus M phase extracts.	bind
9012	2	2799	7	10	NULL	NULL	NULL	IBB	AminoAcid	excess	promotes					microtubule assembly	Process				NULL	Xenopus M phase extracts	NULL	NULL	NULL	NULL	gw60_cell_104_1_83_s_82	11163242	(A) Excess of NLS peptide  and of the importin beta binding fragment of importin   (IBB) promotes microtubule  assembly in  Xenopus M phase extracts.	bind
9013	3	2799	7	10	NULL	NULL	NULL	IBB	AminoAcid		is					importin beta binding fragment of importin	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_104_1_83_s_82	11163242	(A) Excess of NLS peptide  and of the importin beta binding fragment of importin   (IBB) promotes microtubule  assembly in  Xenopus M phase extracts.	bind
5850	1	2800	5	10	NULL	NULL	NULL	SKP1	GP		bind					CUL1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_6_1519_s_168	12504026	(A) Expression of CAND1 prevents SKP1 binding to CUL1.	bind
5851	2	2800	5	10	NULL	NULL	NULL	CAND1	GP	expression	prevent					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_6_1519_s_168	12504026	(A) Expression of CAND1 prevents SKP1 binding to CUL1.	bind
9014	1	2800	7	10	NULL	NULL	NULL	SKP1	GP		bind					CUL1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_6_1519_s_168	12504026	(A) Expression of CAND1 prevents SKP1 binding to CUL1.	bind
9015	2	2800	7	10	NULL	NULL	NULL	CAND1	GP	expression of	prevents					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_6_1519_s_168	12504026	(A) Expression of CAND1 prevents SKP1 binding to CUL1.	bind
6062	2	2802	5	10	NULL	NULL	NULL	13C4 mAb	GP		inhibit			Fab-fragment		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_8_2453_s_150	11514628	(A) Fab-fragment of 13C4 mAb inhibits STxB binding to Gb3.	bind
6063	1	2802	5	10	NULL	NULL	NULL	STxB	GP		bind					Gb3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_8_2453_s_150	11514628	(A) Fab-fragment of 13C4 mAb inhibits STxB binding to Gb3.	bind
6045	1	2802	6	10	NULL	NULL	NULL	STxB 	GP		bind					Gb3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_8_2453_s_150	11514628	(A) Fab-fragment of 13C4 mAb inhibits STxB binding to Gb3.	bind
6046	2	2802	6	10	NULL	NULL	NULL	13C4 mAb	GP		inhibits			Fab-fragment		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_8_2453_s_150	11514628	(A) Fab-fragment of 13C4 mAb inhibits STxB binding to Gb3.	bind
6064	1	2803	5	10	NULL	NULL	NULL	CPSF	GP		bind					GST-TFIIS	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_6154_s_174	10454562	(A) factors CPSF and CstF bound to GST-TFIIS ( 41) but not to GST-VP16.	bind
6065	2	2803	5	10	NULL	NULL	NULL	CstF	GP		bind					GST-TFIIS	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_6154_s_174	10454562	(A) factors CPSF and CstF bound to GST-TFIIS ( 41) but not to GST-VP16.	bind
6066	3	2803	5	10	NULL	NULL	NULL	CPSF	GP		does not bind					GST-VP16	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_6154_s_174	10454562	(A) factors CPSF and CstF bound to GST-TFIIS ( 41) but not to GST-VP16.	bind
6067	4	2803	5	10	NULL	NULL	NULL	CstF	GP		does not bind					GST-VP16	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_6154_s_174	10454562	(A) factors CPSF and CstF bound to GST-TFIIS ( 41) but not to GST-VP16.	bind
6047	1	2803	6	10	NULL	NULL	NULL	CPSF	GP		bind					GST-TFIIS	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_6154_s_174	10454562	(A) factors CPSF and CstF bound to GST-TFIIS ( 41) but not to GST-VP16.	bind
6048	2	2803	6	10	NULL	NULL	NULL	CstF	GP		bind					GST-TFIIS	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_6154_s_174	10454562	(A) factors CPSF and CstF bound to GST-TFIIS ( 41) but not to GST-VP16.	bind
6049	3	2803	6	10	NULL	NULL	NULL	CPSF	GP		does not bind					GST-VP16	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_6154_s_174	10454562	(A) factors CPSF and CstF bound to GST-TFIIS ( 41) but not to GST-VP16.	bind
6050	4	2803	6	10	NULL	NULL	NULL	CstF	GP		does not bind					GST-VP16	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_6154_s_174	10454562	(A) factors CPSF and CstF bound to GST-TFIIS ( 41) but not to GST-VP16.	bind
6068	1	2804	5	10	NULL	NULL	NULL	Fibulin-1	GP		bind					BPV-1 E6	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_4_962_s_112	12200142	(A) Fibulin-1 binds to BPV-1 E6 and HPV-16 E6.	bind
6069	2	2804	5	10	NULL	NULL	NULL	Fibulin-1	GP		bind					HPV-16 E6	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_4_962_s_112	12200142	(A) Fibulin-1 binds to BPV-1 E6 and HPV-16 E6.	bind
6051	1	2804	6	10	NULL	NULL	NULL	Fibulin-1	GP		bind					BPV-1 E6	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_4_962_s_112	12200142	(A) Fibulin-1 binds to BPV-1 E6 and HPV-16 E6.	bind
6052	2	2804	6	10	NULL	NULL	NULL	Fibulin-1	GP		bind					HPV-16 E6	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_4_962_s_112	12200142	(A) Fibulin-1 binds to BPV-1 E6 and HPV-16 E6.	bind
6070	1	2805	5	10	NULL	NULL	NULL	PSC	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_3_545_s_136	11583617	(A) Filter binding assay for binding of PSC (top panel) and PCC (bottom panel) to DNA.	bind
6071	2	2805	5	10	NULL	NULL	NULL	PCC	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_3_545_s_136	11583617	(A) Filter binding assay for binding of PSC (top panel) and PCC (bottom panel) to DNA.	bind
6053	1	2805	6	10	NULL	NULL	NULL	PSC	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_3_545_s_136	11583617	(A) Filter binding assay for binding of PSC (top panel) and PCC (bottom panel) to DNA.	bind
6054	2	2805	6	10	NULL	NULL	NULL	PCC	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_3_545_s_136	11583617	(A) Filter binding assay for binding of PSC (top panel) and PCC (bottom panel) to DNA.	bind
6072	1	2808	5	10	NULL	NULL	NULL	diazepam	Chemical		bind					HSA	GP	native			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1750_1_93_s_168	15890566	(A) Fluorescence quench titration results of diazepam binding to native HSA  ( ) and HSA denatured with 1.0 M ( ) 1.8 M ( ) and 6.0 M ( ) GnHCl concentration.	bind
6073	2	2808	5	10	NULL	NULL	NULL	diazepam	Chemical		bind					HSA	GP	denatured			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1750_1_93_s_168	15890566	(A) Fluorescence quench titration results of diazepam binding to native HSA  ( ) and HSA denatured with 1.0 M ( ) 1.8 M ( ) and 6.0 M ( ) GnHCl concentration.	bind
53054	3	2808	5	10	NULL	NULL	NULL	GnHCl	Chemical		denatures					HSA	GP	native			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1750_1_93_s_168	15890566	(A) Fluorescence quench titration results of diazepam binding to native HSA  ( ) and HSA denatured with 1.0 M ( ) 1.8 M ( ) and 6.0 M ( ) GnHCl concentration.	bind
6055	1	2808	6	10	NULL	NULL	NULL	diazepam	Chemical		bind					HSA	GP	native			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1750_1_93_s_168	15890566	(A) Fluorescence quench titration results of diazepam binding to native HSA  ( ) and HSA denatured with 1.0 M ( ) 1.8 M ( ) and 6.0 M ( ) GnHCl concentration.	bind
6056	2	2808	6	10	NULL	NULL	NULL	diazepam	Chemical		bind					HSA	GP	denatured			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1750_1_93_s_168	15890566	(A) Fluorescence quench titration results of diazepam binding to native HSA  ( ) and HSA denatured with 1.0 M ( ) 1.8 M ( ) and 6.0 M ( ) GnHCl concentration.	bind
6057	3	2808	6	10	NULL	NULL	NULL	GnHCl	Chemical		denatures					HSA	GP	native			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1750_1_93_s_168	15890566	(A) Fluorescence quench titration results of diazepam binding to native HSA  ( ) and HSA denatured with 1.0 M ( ) 1.8 M ( ) and 6.0 M ( ) GnHCl concentration.	bind
6074	1	2809	5	10	NULL	NULL	NULL	SarA	GP		bind					sarV	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_16_5267_s_186	15292128	(A) Footprint analysis of SarA binding to the  sarV promoter region.	bind
6058	1	2809	6	10	NULL	NULL	NULL	SarA	GP		bind					sarV	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_16_5267_s_186	15292128	(A) Footprint analysis of SarA binding to the  sarV promoter region.	bind
6075	1	2811	5	NULL	NULL	0	NULL		NULL	free	bind	NULL		N1-22			NULL		N1-22		NULL		0	NULL	NULL	NULL	gw60_molcell_1_2_265_s_45	9659923	(A) free N1-22, (B) free  boxB RNA, and  boxB RNA bound to (C) N1-22, (D) N1-47, and (E) the full-length N protein.	bind
6076	2	2811	5	NULL	NULL	0	NULL		NULL	free	bind	NULL		N1-22			NULL		N1-47		NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_265_s_45	9659923	(A) free N1-22, (B) free  boxB RNA, and  boxB RNA bound to (C) N1-22, (D) N1-47, and (E) the full-length N protein.	bind
6077	3	2811	5	10	NULL	NULL	NULL			free	bind			N1-22		N protein	GP	full-length			NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_265_s_45	9659923	(A) free N1-22, (B) free  boxB RNA, and  boxB RNA bound to (C) N1-22, (D) N1-47, and (E) the full-length N protein.	bind
6078	4	2811	5	10	NULL	NULL	NULL	RNA	NucleicAcid	free	bind				boxB				N1-22		NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_265_s_45	9659923	(A) free N1-22, (B) free  boxB RNA, and  boxB RNA bound to (C) N1-22, (D) N1-47, and (E) the full-length N protein.	bind
6079	5	2811	5	10	NULL	NULL	NULL	RNA	NucleicAcid	free	bind				boxB				N1-47		NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_265_s_45	9659923	(A) free N1-22, (B) free  boxB RNA, and  boxB RNA bound to (C) N1-22, (D) N1-47, and (E) the full-length N protein.	bind
6080	6	2811	5	10	NULL	NULL	NULL	RNA	NucleicAcid	free	bind				boxB	N protein	GP	full-length			NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_265_s_45	9659923	(A) free N1-22, (B) free  boxB RNA, and  boxB RNA bound to (C) N1-22, (D) N1-47, and (E) the full-length N protein.	bind
6081	7	2811	5	10	NULL	NULL	NULL	RNA	NucleicAcid		bind				boxB				N1-22		NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_265_s_45	9659923	(A) free N1-22, (B) free  boxB RNA, and  boxB RNA bound to (C) N1-22, (D) N1-47, and (E) the full-length N protein.	bind
6082	8	2811	5	10	NULL	NULL	NULL	RNA	NucleicAcid		bind				boxB				N1-47		NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_265_s_45	9659923	(A) free N1-22, (B) free  boxB RNA, and  boxB RNA bound to (C) N1-22, (D) N1-47, and (E) the full-length N protein.	bind
6083	9	2811	5	10	NULL	NULL	NULL	RNA	NucleicAcid		bind				boxB	N protein	GP	full-length			NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_265_s_45	9659923	(A) free N1-22, (B) free  boxB RNA, and  boxB RNA bound to (C) N1-22, (D) N1-47, and (E) the full-length N protein.	bind
6225	1	2811	6	10	NULL	NULL	NULL	RNA	NucleicAcid		bind				boxB				N1-22		NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_265_s_45	9659923	(A) free N1-22, (B) free  boxB RNA, and  boxB RNA bound to (C) N1-22, (D) N1-47, and (E) the full-length N protein.	bind
6226	2	2811	6	10	NULL	NULL	NULL	RNA	NucleicAcid		bind				boxB				N1-47		NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_265_s_45	9659923	(A) free N1-22, (B) free  boxB RNA, and  boxB RNA bound to (C) N1-22, (D) N1-47, and (E) the full-length N protein.	bind
6227	3	2811	6	10	NULL	NULL	NULL	RNA	NucleicAcid		bind				boxB	N protein	GP	full length			NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_265_s_45	9659923	(A) free N1-22, (B) free  boxB RNA, and  boxB RNA bound to (C) N1-22, (D) N1-47, and (E) the full-length N protein.	bind
7272	4	2811	6	NULL	NULL	0	NULL		NULL	free	bind	NULL		N1-22			NULL		N1-22		NULL		0	NULL	NULL	NULL	gw60_molcell_1_2_265_s_45	9659923	(A) free N1-22, (B) free  boxB RNA, and  boxB RNA bound to (C) N1-22, (D) N1-47, and (E) the full-length N protein.	bind
7273	5	2811	6	NULL	NULL	0	NULL		NULL	free	bind	NULL		N1-22			NULL		N1-47		NULL		0	NULL	NULL	NULL	gw60_molcell_1_2_265_s_45	9659923	(A) free N1-22, (B) free  boxB RNA, and  boxB RNA bound to (C) N1-22, (D) N1-47, and (E) the full-length N protein.	bind
7274	6	2811	6	10	NULL	NULL	NULL			free	bind			N1-22		N protein	GP	full length			NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_265_s_45	9659923	(A) free N1-22, (B) free  boxB RNA, and  boxB RNA bound to (C) N1-22, (D) N1-47, and (E) the full-length N protein.	bind
7275	7	2811	6	10	NULL	NULL	NULL	RNA	NucleicAcid	free	bind				boxB				N1-22		NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_265_s_45	9659923	(A) free N1-22, (B) free  boxB RNA, and  boxB RNA bound to (C) N1-22, (D) N1-47, and (E) the full-length N protein.	bind
7276	8	2811	6	10	NULL	NULL	NULL	RNA	NucleicAcid	free	bind				boxB				N1-47		NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_265_s_45	9659923	(A) free N1-22, (B) free  boxB RNA, and  boxB RNA bound to (C) N1-22, (D) N1-47, and (E) the full-length N protein.	bind
53055	9	2811	6	10	NULL	NULL	NULL	 RNA	NucleicAcid	free	bind				boxB	N protein	GP	full-length			NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_265_s_45	9659923	(A) free N1-22, (B) free  boxB RNA, and  boxB RNA bound to (C) N1-22, (D) N1-47, and (E) the full-length N protein.	bind
6084	1	2814	5	10	NULL	NULL	NULL	GATA3	GP		bind					RALDH2-T	GP			GATA site in the promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6939_s_225	9819382	(A) GATA3 binds to the GATA site in the RALDH2-T promoter.	bind
6059	1	2814	6	10	NULL	NULL	NULL	GATA3	GP		bind					RALDH2-T	GP			GATA site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6939_s_225	9819382	(A) GATA3 binds to the GATA site in the RALDH2-T promoter.	bind
6085	1	2815	5	10	NULL	NULL	NULL	Gcn4	GP		bind									GCREs	NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_6_1309_s_131	11163205	(A) Gcn4 binds GCREs independently of Gcn5.	bind
6086	2	2815	5	10	NULL	NULL	NULL	statement 1	Process		is independent of					Gcn5	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_6_1309_s_131	11163205	(A) Gcn4 binds GCREs independently of Gcn5.	bind
6060	1	2815	6	10	NULL	NULL	NULL	Gcn4	GP		bind									GCRE	NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_6_1309_s_131	11163205	(A) Gcn4 binds GCREs independently of Gcn5.	bind
6061	2	2815	6	10	NULL	NULL	NULL	statement 1	Process		is independent of					Gcn5	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_6_1309_s_131	11163205	(A) Gcn4 binds GCREs independently of Gcn5.	bind
6087	1	2816	5	10	NULL	NULL	NULL	NFATp	GP	purified;;recombinant	bind					IL-3	GP			NFAT-like elements in enhancer	NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_2_175_s_145	9047239	(A) Gel electrophoretic mobility shift assays of purified recombinant NFATp and AP-1 binding to NFAT-like elements in the IL-3 enhancer.	bind
6088	2	2816	5	10	NULL	NULL	NULL	AP-1	GP	purified;;recombinant	bind					IL-3	GP			NFAT-like elements in enhancer	NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_2_175_s_145	9047239	(A) Gel electrophoretic mobility shift assays of purified recombinant NFATp and AP-1 binding to NFAT-like elements in the IL-3 enhancer.	bind
6228	1	2816	6	10	NULL	NULL	NULL	NFATp	GP	purified;;recombinant	bind					IL-3	GP			NFAT-like elements in enhancer	NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_2_175_s_145	9047239	(A) Gel electrophoretic mobility shift assays of purified recombinant NFATp and AP-1 binding to NFAT-like elements in the IL-3 enhancer.	bind
6229	2	2816	6	10	NULL	NULL	NULL	AP-1	GP	purified;;recombinant	bind					IL-3	GP			NFAT-like elements in enhancer	NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_2_175_s_145	9047239	(A) Gel electrophoretic mobility shift assays of purified recombinant NFATp and AP-1 binding to NFAT-like elements in the IL-3 enhancer.	bind
6089	1	2817	5	10	NULL	NULL	NULL	Tead2	GP		bind									CE	NULL		NULL	NULL	NULL	NULL	gw70_development_132_21_4719_s_169	16207754	(A) Gel mobility shift assay  showing that Tead2 and Tead4 bind to the CE.	bind
6090	2	2817	5	10	NULL	NULL	NULL	Tead4	GP		bind									CE	NULL		NULL	NULL	NULL	NULL	gw70_development_132_21_4719_s_169	16207754	(A) Gel mobility shift assay  showing that Tead2 and Tead4 bind to the CE.	bind
6230	1	2817	6	10	NULL	NULL	NULL	Tead2	GP		bind									CE	NULL		NULL	NULL	NULL	NULL	gw70_development_132_21_4719_s_169	16207754	(A) Gel mobility shift assay  showing that Tead2 and Tead4 bind to the CE.	bind
6231	2	2817	6	10	NULL	NULL	NULL	Tead4	GP		bind									CE	NULL		NULL	NULL	NULL	NULL	gw70_development_132_21_4719_s_169	16207754	(A) Gel mobility shift assay  showing that Tead2 and Tead4 bind to the CE.	bind
6091	1	2821	5	10	NULL	NULL	NULL	factors			bind					NF- B	GP				NULL	in nuclear extracts from pro-B cells	NULL	NULL	NULL	NULL	gw60_immunity_6_2_131_s_137	9047235	(A) Gel shift analysis of factors in nuclear extracts from pro- and pre-B cells that bind to NF- B or octamer probes.	bind
6092	2	2821	5	10	NULL	NULL	NULL	factors			bind					octamer probes	NucleicAcid				NULL	in nuclear extracts from pro-B cells	NULL	NULL	NULL	NULL	gw60_immunity_6_2_131_s_137	9047235	(A) Gel shift analysis of factors in nuclear extracts from pro- and pre-B cells that bind to NF- B or octamer probes.	bind
6093	3	2821	5	10	NULL	NULL	NULL	factors			bind					NF- B	GP				NULL	in nuclear extracts from pre-B cells	NULL	NULL	NULL	NULL	gw60_immunity_6_2_131_s_137	9047235	(A) Gel shift analysis of factors in nuclear extracts from pro- and pre-B cells that bind to NF- B or octamer probes.	bind
6094	4	2821	5	10	NULL	NULL	NULL	factors			bind					octamer probes	NucleicAcid				NULL	in nuclear extracts from pre-B cells	NULL	NULL	NULL	NULL	gw60_immunity_6_2_131_s_137	9047235	(A) Gel shift analysis of factors in nuclear extracts from pro- and pre-B cells that bind to NF- B or octamer probes.	bind
46516	5	2821	5	10	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_2_131_s_137	9047235	(A) Gel shift analysis of factors in nuclear extracts from pro- and pre-B cells that bind to NF- B or octamer probes.	bind
46517	6	2821	5	10	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_2_131_s_137	9047235	(A) Gel shift analysis of factors in nuclear extracts from pro- and pre-B cells that bind to NF- B or octamer probes.	bind
6232	1	2821	6	10	NULL	NULL	NULL	factor			bind					NF-B 	GP			site	NULL	nuclear extracts from pro-B cells	NULL	NULL	NULL	NULL	gw60_immunity_6_2_131_s_137	9047235	(A) Gel shift analysis of factors in nuclear extracts from pro- and pre-B cells that bind to NF- B or octamer probes.	bind
6233	2	2821	6	10	NULL	NULL	NULL	factor			bind					octamer probe	NucleicAcid			site	NULL	nuclear extracts from pro-B cells	NULL	NULL	NULL	NULL	gw60_immunity_6_2_131_s_137	9047235	(A) Gel shift analysis of factors in nuclear extracts from pro- and pre-B cells that bind to NF- B or octamer probes.	bind
6234	3	2821	6	10	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_2_131_s_137	9047235	(A) Gel shift analysis of factors in nuclear extracts from pro- and pre-B cells that bind to NF- B or octamer probes.	bind
46513	4	2821	6	10	NULL	NULL	NULL	factors			bind					NF-B 	GP				NULL	 in nuclear extracts from pre-B cells	NULL	NULL	NULL	NULL	gw60_immunity_6_2_131_s_137	9047235	(A) Gel shift analysis of factors in nuclear extracts from pro- and pre-B cells that bind to NF- B or octamer probes.	bind
46514	5	2821	6	10	NULL	NULL	NULL	factors			bind					octamer probes	NucleicAcid				NULL	in nuclear extracts from pre-B cells	NULL	NULL	NULL	NULL	gw60_immunity_6_2_131_s_137	9047235	(A) Gel shift analysis of factors in nuclear extracts from pro- and pre-B cells that bind to NF- B or octamer probes.	bind
46515	6	2821	6	10	NULL	NULL	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_2_131_s_137	9047235	(A) Gel shift analysis of factors in nuclear extracts from pro- and pre-B cells that bind to NF- B or octamer probes.	bind
6095	1	2822	5	NULL	NULL	0	NULL		NULL	complete	contain	NULL			127-nt enhancer		NULL	wild-type		pyrimidine tract	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_1_78_s_203	9858533	(A) Gel shift analysis of the binding of PTB (top) and U2AF (bottom) to the 127-nt complete enhancer containing the wild-type pyrimidine tract (wild type), purine mutation (purine), or U2AF mutation (U2AF).	bind
6096	2	2822	5	NULL	NULL	0	NULL		NULL	complete	contain	NULL			127-nt enhancer		NULL	mutant		purine	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_1_78_s_203	9858533	(A) Gel shift analysis of the binding of PTB (top) and U2AF (bottom) to the 127-nt complete enhancer containing the wild-type pyrimidine tract (wild type), purine mutation (purine), or U2AF mutation (U2AF).	bind
6097	3	2822	5	10	NULL	NULL	NULL			complete	contain				127-nt enhancer	U2AF	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_78_s_203	9858533	(A) Gel shift analysis of the binding of PTB (top) and U2AF (bottom) to the 127-nt complete enhancer containing the wild-type pyrimidine tract (wild type), purine mutation (purine), or U2AF mutation (U2AF).	bind
6098	4	2822	5	10	NULL	NULL	NULL	PTB	GP		bind					statement 1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_78_s_203	9858533	(A) Gel shift analysis of the binding of PTB (top) and U2AF (bottom) to the 127-nt complete enhancer containing the wild-type pyrimidine tract (wild type), purine mutation (purine), or U2AF mutation (U2AF).	bind
6099	5	2822	5	10	NULL	NULL	NULL	PTB	GP		bind					statement 2	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_78_s_203	9858533	(A) Gel shift analysis of the binding of PTB (top) and U2AF (bottom) to the 127-nt complete enhancer containing the wild-type pyrimidine tract (wild type), purine mutation (purine), or U2AF mutation (U2AF).	bind
6100	6	2822	5	10	NULL	NULL	NULL	PTB	GP		bind					statement 3	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_78_s_203	9858533	(A) Gel shift analysis of the binding of PTB (top) and U2AF (bottom) to the 127-nt complete enhancer containing the wild-type pyrimidine tract (wild type), purine mutation (purine), or U2AF mutation (U2AF).	bind
6101	7	2822	5	10	NULL	NULL	NULL	statement 4	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_78_s_203	9858533	(A) Gel shift analysis of the binding of PTB (top) and U2AF (bottom) to the 127-nt complete enhancer containing the wild-type pyrimidine tract (wild type), purine mutation (purine), or U2AF mutation (U2AF).	bind
6102	8	2822	5	10	NULL	NULL	NULL	statement 5	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_78_s_203	9858533	(A) Gel shift analysis of the binding of PTB (top) and U2AF (bottom) to the 127-nt complete enhancer containing the wild-type pyrimidine tract (wild type), purine mutation (purine), or U2AF mutation (U2AF).	bind
6103	9	2822	5	10	NULL	NULL	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_78_s_203	9858533	(A) Gel shift analysis of the binding of PTB (top) and U2AF (bottom) to the 127-nt complete enhancer containing the wild-type pyrimidine tract (wild type), purine mutation (purine), or U2AF mutation (U2AF).	bind
6104	10	2822	5	10	NULL	NULL	NULL	U2AF	GP		bind					statement 1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_78_s_203	9858533	(A) Gel shift analysis of the binding of PTB (top) and U2AF (bottom) to the 127-nt complete enhancer containing the wild-type pyrimidine tract (wild type), purine mutation (purine), or U2AF mutation (U2AF).	bind
6105	11	2822	5	10	NULL	NULL	NULL	U2AF	GP		bind					statement 2	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_78_s_203	9858533	(A) Gel shift analysis of the binding of PTB (top) and U2AF (bottom) to the 127-nt complete enhancer containing the wild-type pyrimidine tract (wild type), purine mutation (purine), or U2AF mutation (U2AF).	bind
6106	12	2822	5	10	NULL	NULL	NULL	U2AF	GP		bind					statement 3	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_78_s_203	9858533	(A) Gel shift analysis of the binding of PTB (top) and U2AF (bottom) to the 127-nt complete enhancer containing the wild-type pyrimidine tract (wild type), purine mutation (purine), or U2AF mutation (U2AF).	bind
6107	13	2822	5	10	NULL	NULL	NULL	statement 10	Process		is an alternative to					statement 11	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_78_s_203	9858533	(A) Gel shift analysis of the binding of PTB (top) and U2AF (bottom) to the 127-nt complete enhancer containing the wild-type pyrimidine tract (wild type), purine mutation (purine), or U2AF mutation (U2AF).	bind
6108	14	2822	5	10	NULL	NULL	NULL	statement 10	Process		is an alternative to					statement 12	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_78_s_203	9858533	(A) Gel shift analysis of the binding of PTB (top) and U2AF (bottom) to the 127-nt complete enhancer containing the wild-type pyrimidine tract (wild type), purine mutation (purine), or U2AF mutation (U2AF).	bind
6109	15	2822	5	10	NULL	NULL	NULL	statement 11	Process		is an alternative to					statement 12	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_78_s_203	9858533	(A) Gel shift analysis of the binding of PTB (top) and U2AF (bottom) to the 127-nt complete enhancer containing the wild-type pyrimidine tract (wild type), purine mutation (purine), or U2AF mutation (U2AF).	bind
6235	1	2822	6	10	NULL	NULL	NULL			complete	contains				 127-nt enhancer 	pyrimidine tract	NucleicAcid	wild type			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_78_s_203	9858533	(A) Gel shift analysis of the binding of PTB (top) and U2AF (bottom) to the 127-nt complete enhancer containing the wild-type pyrimidine tract (wild type), purine mutation (purine), or U2AF mutation (U2AF).	bind
6236	2	2822	6	10	NULL	NULL	NULL			complete	contains				127-nt enhancer	purine	NucleicAcid	mutant			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_78_s_203	9858533	(A) Gel shift analysis of the binding of PTB (top) and U2AF (bottom) to the 127-nt complete enhancer containing the wild-type pyrimidine tract (wild type), purine mutation (purine), or U2AF mutation (U2AF).	bind
6237	3	2822	6	10	NULL	NULL	NULL			complete	contains				127-nt enhancer	U2AF	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_78_s_203	9858533	(A) Gel shift analysis of the binding of PTB (top) and U2AF (bottom) to the 127-nt complete enhancer containing the wild-type pyrimidine tract (wild type), purine mutation (purine), or U2AF mutation (U2AF).	bind
6238	4	2822	6	10	NULL	NULL	NULL	U2AF	GP		bind					statement 1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_78_s_203	9858533	(A) Gel shift analysis of the binding of PTB (top) and U2AF (bottom) to the 127-nt complete enhancer containing the wild-type pyrimidine tract (wild type), purine mutation (purine), or U2AF mutation (U2AF).	bind
6905	5	2822	6	10	NULL	NULL	NULL	U2AF	GP		bind					statement 2	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_78_s_203	9858533	(A) Gel shift analysis of the binding of PTB (top) and U2AF (bottom) to the 127-nt complete enhancer containing the wild-type pyrimidine tract (wild type), purine mutation (purine), or U2AF mutation (U2AF).	bind
6906	6	2822	6	10	NULL	NULL	NULL	U2AF	GP		bind					statement 3	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_78_s_203	9858533	(A) Gel shift analysis of the binding of PTB (top) and U2AF (bottom) to the 127-nt complete enhancer containing the wild-type pyrimidine tract (wild type), purine mutation (purine), or U2AF mutation (U2AF).	bind
6907	7	2822	6	10	NULL	NULL	NULL	PTB	GP		bind					statement 1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_78_s_203	9858533	(A) Gel shift analysis of the binding of PTB (top) and U2AF (bottom) to the 127-nt complete enhancer containing the wild-type pyrimidine tract (wild type), purine mutation (purine), or U2AF mutation (U2AF).	bind
46886	8	2822	6	10	NULL	NULL	NULL	PTB	GP		bind					statement 2	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_78_s_203	9858533	(A) Gel shift analysis of the binding of PTB (top) and U2AF (bottom) to the 127-nt complete enhancer containing the wild-type pyrimidine tract (wild type), purine mutation (purine), or U2AF mutation (U2AF).	bind
46887	9	2822	6	10	NULL	NULL	NULL	PTB	GP		bind					statement 3	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_78_s_203	9858533	(A) Gel shift analysis of the binding of PTB (top) and U2AF (bottom) to the 127-nt complete enhancer containing the wild-type pyrimidine tract (wild type), purine mutation (purine), or U2AF mutation (U2AF).	bind
53065	10	2822	6	10	NULL	NULL	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_78_s_203	9858533	(A) Gel shift analysis of the binding of PTB (top) and U2AF (bottom) to the 127-nt complete enhancer containing the wild-type pyrimidine tract (wild type), purine mutation (purine), or U2AF mutation (U2AF).	bind
53066	11	2822	6	10	NULL	NULL	NULL	statement 4	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_78_s_203	9858533	(A) Gel shift analysis of the binding of PTB (top) and U2AF (bottom) to the 127-nt complete enhancer containing the wild-type pyrimidine tract (wild type), purine mutation (purine), or U2AF mutation (U2AF).	bind
53067	12	2822	6	10	NULL	NULL	NULL	statement 5	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_78_s_203	9858533	(A) Gel shift analysis of the binding of PTB (top) and U2AF (bottom) to the 127-nt complete enhancer containing the wild-type pyrimidine tract (wild type), purine mutation (purine), or U2AF mutation (U2AF).	bind
53068	13	2822	6	10	NULL	NULL	NULL	statement 7	Process		is an alternative to					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_78_s_203	9858533	(A) Gel shift analysis of the binding of PTB (top) and U2AF (bottom) to the 127-nt complete enhancer containing the wild-type pyrimidine tract (wild type), purine mutation (purine), or U2AF mutation (U2AF).	bind
53069	14	2822	6	10	NULL	NULL	NULL	statement 7	Process		is an alternative to					statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_78_s_203	9858533	(A) Gel shift analysis of the binding of PTB (top) and U2AF (bottom) to the 127-nt complete enhancer containing the wild-type pyrimidine tract (wild type), purine mutation (purine), or U2AF mutation (U2AF).	bind
53070	15	2822	6	10	NULL	NULL	NULL	statement 8	Process		is an alternative to					statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_78_s_203	9858533	(A) Gel shift analysis of the binding of PTB (top) and U2AF (bottom) to the 127-nt complete enhancer containing the wild-type pyrimidine tract (wild type), purine mutation (purine), or U2AF mutation (U2AF).	bind
6110	1	2823	5	10	NULL	NULL	NULL	CcpA	GP		is in complex with					HPr	GP		Ser-P		NULL		NULL	NULL	NULL	NULL	gw70_applenvironmicrob_70_9_5244_s_188	15345406	(A) Gel shift assay showing the binding of the complex consisting of CcpA  and HPr-[Ser-P] to the  cre site.	bind
6111	2	2823	5	10	NULL	NULL	NULL	statement 1	Process		bind									cre site	NULL		NULL	NULL	NULL	NULL	gw70_applenvironmicrob_70_9_5244_s_188	15345406	(A) Gel shift assay showing the binding of the complex consisting of CcpA  and HPr-[Ser-P] to the  cre site.	bind
6240	1	2823	6	10	NULL	NULL	NULL	CcpA	GP		forms a complex with					HPr	GP		Ser-P		NULL		NULL	NULL	NULL	NULL	gw70_applenvironmicrob_70_9_5244_s_188	15345406	(A) Gel shift assay showing the binding of the complex consisting of CcpA  and HPr-[Ser-P] to the  cre site.	bind
6242	2	2823	6	10	NULL	NULL	NULL	statement 1	Process		bind									cre site	NULL		NULL	NULL	NULL	NULL	gw70_applenvironmicrob_70_9_5244_s_188	15345406	(A) Gel shift assay showing the binding of the complex consisting of CcpA  and HPr-[Ser-P] to the  cre site.	bind
6112	1	2824	5	10	NULL	NULL	NULL	TR	GP		bind					PGDS	GP			T3RE	NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_55_2_321_s_133	9582446	(A) Gel-shift assay showing the binding properties of TR to the PGDS-T3RE.	bind
6244	1	2824	6	10	NULL	NULL	NULL	TR	GP		bind					PGDS	GP			T3RE	NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_55_2_321_s_133	9582446	(A) Gel-shift assay showing the binding properties of TR to the PGDS-T3RE.	bind
6113	1	2825	5	10	NULL	NULL	NULL	Tem1	GP		bind					Bub2	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_219_s_172	14734533	(A) Gic1 disrupts the binding between Tem1 and Bub2.	bind
6115	2	2825	5	10	NULL	NULL	NULL	Gic1	GP		disrupt					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_219_s_172	14734533	(A) Gic1 disrupts the binding between Tem1 and Bub2.	bind
6245	1	2825	6	10	NULL	NULL	NULL	Tem1	GP		bind					Bub2	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_219_s_172	14734533	(A) Gic1 disrupts the binding between Tem1 and Bub2.	bind
6246	2	2825	6	10	NULL	NULL	NULL	Gic1	GP		disrupts					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_219_s_172	14734533	(A) Gic1 disrupts the binding between Tem1 and Bub2.	bind
6116	1	2826	5	10	NULL	NULL	NULL	GrB-OG	GP		bind					CI-MPR+ cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_3_491_s_84	11081635	(A) GrB-OG  binding to CI-MPR+ cells in the presence or absence of M6P or  D-mannose at different concentrations, or with 50 mM D-glucose or D-glucose-6 phosphate.	bind
6247	1	2826	6	10	NULL	NULL	NULL	GrB-OG	GP		bind					CI-MPR+ cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_3_491_s_84	11081635	(A) GrB-OG  binding to CI-MPR+ cells in the presence or absence of M6P or  D-mannose at different concentrations, or with 50 mM D-glucose or D-glucose-6 phosphate.	bind
6129	1	2828	5	10	NULL	NULL	NULL	ankyrin B	GP		bind					L1-CAM	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_6_2696_s_232	16597699	(A) Growth-factor inhibition of ankyrin B binding to L1-CAM is dependent  on activation of the MAPK pathway.	bind
6130	2	2828	5	10	NULL	NULL	NULL	growth-factor	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_6_2696_s_232	16597699	(A) Growth-factor inhibition of ankyrin B binding to L1-CAM is dependent  on activation of the MAPK pathway.	bind
6131	3	2828	5	10	NULL	NULL	NULL	statement 2	Process		is dependent on					MAPK pathway	Process	activation of 			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_6_2696_s_232	16597699	(A) Growth-factor inhibition of ankyrin B binding to L1-CAM is dependent  on activation of the MAPK pathway.	bind
6250	1	2828	6	10	NULL	NULL	NULL	ankyrin B	GP		bind					L1-CAM	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_6_2696_s_232	16597699	(A) Growth-factor inhibition of ankyrin B binding to L1-CAM is dependent  on activation of the MAPK pathway.	bind
6255	2	2828	6	10	NULL	NULL	NULL	growth factor	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_6_2696_s_232	16597699	(A) Growth-factor inhibition of ankyrin B binding to L1-CAM is dependent  on activation of the MAPK pathway.	bind
6256	3	2828	6	10	NULL	NULL	NULL	statement 2	Process		is dependent on					MAPK pathway	Process	activation of			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_6_2696_s_232	16597699	(A) Growth-factor inhibition of ankyrin B binding to L1-CAM is dependent  on activation of the MAPK pathway.	bind
6134	1	2848	5	10	NULL	NULL	NULL	GST-p300	GP		bind					Cdk2	GP	from nuclear extracts			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_157	10330164	(A) GST-p300 binds Cdk2 from nuclear extracts.	bind
6258	1	2848	6	10	NULL	NULL	NULL	GST-p300	GP		bind					Cdk2	GP	nuclear extracts			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_157	10330164	(A) GST-p300 binds Cdk2 from nuclear extracts.	bind
6135	1	2851	5	10	NULL	NULL	NULL	ARF1t	GP	human	bind					coatomer	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_96_6_893_s_44	10102276	(A) GTP-dependent binding  of human ARF1t to coatomer.	bind
6136	2	2851	5	10	NULL	NULL	NULL	statement 1	Process		is dependent on					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_96_6_893_s_44	10102276	(A) GTP-dependent binding  of human ARF1t to coatomer.	bind
6259	1	2851	6	10	NULL	NULL	NULL	ARF1t	GP	human	bind					coatomer	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_96_6_893_s_44	10102276	(A) GTP-dependent binding  of human ARF1t to coatomer.	bind
6260	2	2851	6	10	NULL	NULL	NULL	statement 1	Process		is dependent on					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_96_6_893_s_44	10102276	(A) GTP-dependent binding  of human ARF1t to coatomer.	bind
6137	1	2852	5	10	NULL	NULL	NULL	DRIP205	GP		bind					PPARgamma-RXR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_21_8008_s_134	11027271	(A) GW1929 titration of DRIP205 binding to PPARgamma-RXR.	bind
6261	1	2852	6	10	NULL	NULL	NULL	DRIP205	GP		bind					PPARgamma-RXR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_21_8008_s_134	11027271	(A) GW1929 titration of DRIP205 binding to PPARgamma-RXR.	bind
6138	1	2853	5	10	NULL	NULL	NULL	H1	AminoAcid		bind					GDP-like (Taxol) microtubules	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_11_5373_s_161	16120651	(A) H1 binds GDP-like (Taxol)  microtubules with a 0.67  plus-or-minus  0.08 muM affinity; (B) H1 binds GTP-like  (GMPCPP) microtubules with a 0.40  plus-or-minus  0.05 muM affinity; (C) H1 binds  GTP tubulin with a 0.26  plus-or-minus  0.04 muM affinity; (D) binding kinetics were  studied by adding tubulin (1 muM, blue); 2 muM, red; or 4 muM green) to labeled H1.	bind
6139	2	2853	5	10	NULL	NULL	NULL	H1	AminoAcid		bind					GTP-like (GMPCPP) microtubules	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_11_5373_s_161	16120651	(A) H1 binds GDP-like (Taxol)  microtubules with a 0.67  plus-or-minus  0.08 muM affinity; (B) H1 binds GTP-like  (GMPCPP) microtubules with a 0.40  plus-or-minus  0.05 muM affinity; (C) H1 binds  GTP tubulin with a 0.26  plus-or-minus  0.04 muM affinity; (D) binding kinetics were  studied by adding tubulin (1 muM, blue); 2 muM, red; or 4 muM green) to labeled H1.	bind
6140	3	2853	5	10	NULL	NULL	NULL	H1	AminoAcid		bind					GTP tubulin	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_11_5373_s_161	16120651	(A) H1 binds GDP-like (Taxol)  microtubules with a 0.67  plus-or-minus  0.08 muM affinity; (B) H1 binds GTP-like  (GMPCPP) microtubules with a 0.40  plus-or-minus  0.05 muM affinity; (C) H1 binds  GTP tubulin with a 0.26  plus-or-minus  0.04 muM affinity; (D) binding kinetics were  studied by adding tubulin (1 muM, blue); 2 muM, red; or 4 muM green) to labeled H1.	bind
6262	1	2853	6	10	NULL	NULL	NULL	H1	AminoAcid		bind					GDP-like (Taxol) microtubules	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_11_5373_s_161	16120651	(A) H1 binds GDP-like (Taxol)  microtubules with a 0.67  plus-or-minus  0.08 muM affinity; (B) H1 binds GTP-like  (GMPCPP) microtubules with a 0.40  plus-or-minus  0.05 muM affinity; (C) H1 binds  GTP tubulin with a 0.26  plus-or-minus  0.04 muM affinity; (D) binding kinetics were  studied by adding tubulin (1 muM, blue); 2 muM, red; or 4 muM green) to labeled H1.	bind
6263	2	2853	6	10	NULL	NULL	NULL	H1	AminoAcid		bind					GTP-like (GMPCPP) microtubules	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_11_5373_s_161	16120651	(A) H1 binds GDP-like (Taxol)  microtubules with a 0.67  plus-or-minus  0.08 muM affinity; (B) H1 binds GTP-like  (GMPCPP) microtubules with a 0.40  plus-or-minus  0.05 muM affinity; (C) H1 binds  GTP tubulin with a 0.26  plus-or-minus  0.04 muM affinity; (D) binding kinetics were  studied by adding tubulin (1 muM, blue); 2 muM, red; or 4 muM green) to labeled H1.	bind
6264	3	2853	6	10	NULL	NULL	NULL	H1	AminoAcid		bind					GTP tubulin	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_11_5373_s_161	16120651	(A) H1 binds GDP-like (Taxol)  microtubules with a 0.67  plus-or-minus  0.08 muM affinity; (B) H1 binds GTP-like  (GMPCPP) microtubules with a 0.40  plus-or-minus  0.05 muM affinity; (C) H1 binds  GTP tubulin with a 0.26  plus-or-minus  0.04 muM affinity; (D) binding kinetics were  studied by adding tubulin (1 muM, blue); 2 muM, red; or 4 muM green) to labeled H1.	bind
6141	1	2855	5	10	NULL	NULL	NULL	Nup53	GP		bind					FG-nups	GP	subset of			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_5_2382_s_157	15703211	(A) HeLa cells were processed for immunofluorescence  microscopy and probed with affinity-purified rabbit antibodies directed against a  putative vertebrate counterpart of Nup53 and a mouse mAb (mAb414) that binds a subset  of FG-nups.	bind
6142	2	2855	5	10	NULL	NULL	NULL	mAb414	GP	mouse	bind					FG-nups	GP	subset of			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_5_2382_s_157	15703211	(A) HeLa cells were processed for immunofluorescence  microscopy and probed with affinity-purified rabbit antibodies directed against a  putative vertebrate counterpart of Nup53 and a mouse mAb (mAb414) that binds a subset  of FG-nups.	bind
6265	1	2855	6	10	NULL	NULL	NULL	mAb414	GP	mouse	bind					FG-nups	GP	subset of 			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_5_2382_s_157	15703211	(A) HeLa cells were processed for immunofluorescence  microscopy and probed with affinity-purified rabbit antibodies directed against a  putative vertebrate counterpart of Nup53 and a mouse mAb (mAb414) that binds a subset  of FG-nups.	bind
46521	2	2855	6	10	NULL	NULL	NULL	Nup53	GP		bind					FG-nups	GP	subset of			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_5_2382_s_157	15703211	(A) HeLa cells were processed for immunofluorescence  microscopy and probed with affinity-purified rabbit antibodies directed against a  putative vertebrate counterpart of Nup53 and a mouse mAb (mAb414) that binds a subset  of FG-nups.	bind
6143	1	2858	5	10	NULL	NULL	NULL	CBP	GP		bind		high affinity			p65	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_277_s_139	9659924	(A) High-affinity binding of CBP with p65 requires the synergism-specific domain.	bind
6144	2	2858	5	10	NULL	NULL	NULL	statement 1	Process		require								synergism-specific domain		NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_277_s_139	9659924	(A) High-affinity binding of CBP with p65 requires the synergism-specific domain.	bind
6291	1	2858	6	10	NULL	NULL	NULL	CBP	GP		bind					p65	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_277_s_139	9659924	(A) High-affinity binding of CBP with p65 requires the synergism-specific domain.	bind
7277	2	2858	6	10	NULL	NULL	NULL	statement 1	Process		require								synergism-specific domain		NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_277_s_139	9659924	(A) High-affinity binding of CBP with p65 requires the synergism-specific domain.	bind
6145	1	2859	5	10	NULL	NULL	NULL	His6NSF	GP		bind					GST-GluR2	GP		C terminus		NULL		NULL	NULL	NULL	NULL	gw60_neuron_34_1_53_s_51	11931741	(A) His6NSF binding to GST-GluR2 C terminus (R2C) is sensitive to ATP hydrolysis.	bind
6146	2	2859	5	10	NULL	NULL	NULL	statement 1	Process		is sensitive to					ATP 	Chemical	hydrolysis of			NULL		NULL	NULL	NULL	NULL	gw60_neuron_34_1_53_s_51	11931741	(A) His6NSF binding to GST-GluR2 C terminus (R2C) is sensitive to ATP hydrolysis.	bind
46522	3	2859	5	10	NULL	NULL	NULL	R2C	GP		is					GST-GluR2	GP		C terminus		NULL		NULL	NULL	NULL	NULL	gw60_neuron_34_1_53_s_51	11931741	(A) His6NSF binding to GST-GluR2 C terminus (R2C) is sensitive to ATP hydrolysis.	bind
6300	1	2859	6	10	NULL	NULL	NULL	His6NSF	GP		bind					GST-GluR2	GP		 C terminus		NULL		NULL	NULL	NULL	NULL	gw60_neuron_34_1_53_s_51	11931741	(A) His6NSF binding to GST-GluR2 C terminus (R2C) is sensitive to ATP hydrolysis.	bind
6302	2	2859	6	10	NULL	NULL	NULL	statement 1	Process		is sensitive to 					ATP	Chemical	hydrolysis of			NULL		NULL	NULL	NULL	NULL	gw60_neuron_34_1_53_s_51	11931741	(A) His6NSF binding to GST-GluR2 C terminus (R2C) is sensitive to ATP hydrolysis.	bind
46524	3	2859	6	10	NULL	NULL	NULL	R2C	GP		is					GST-GluR2	GP		C terminus		NULL		NULL	NULL	NULL	NULL	gw60_neuron_34_1_53_s_51	11931741	(A) His6NSF binding to GST-GluR2 C terminus (R2C) is sensitive to ATP hydrolysis.	bind
6147	1	2860	5	10	NULL	NULL	NULL	FW	Chemical		bind					AMPA receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_133_7_1055_s_105	11487516	(A) Histogram showing the concentration curve for AChE enhancement of [3]-FW binding to AMPA receptors solubilized with 1% octylglucopyranoside There was a significant increase ( P<0.01, non paired Student's  t-test) in binding to AChE-treated solubilized compared to solubilized control samples.	bind
6148	2	2860	5	10	NULL	NULL	NULL	AChE	GP		enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_133_7_1055_s_105	11487516	(A) Histogram showing the concentration curve for AChE enhancement of [3]-FW binding to AMPA receptors solubilized with 1% octylglucopyranoside There was a significant increase ( P<0.01, non paired Student's  t-test) in binding to AChE-treated solubilized compared to solubilized control samples.	bind
6303	1	2860	6	10	NULL	NULL	NULL	FW	Chemical		bind					AMPA receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_133_7_1055_s_105	11487516	(A) Histogram showing the concentration curve for AChE enhancement of [3]-FW binding to AMPA receptors solubilized with 1% octylglucopyranoside There was a significant increase ( P<0.01, non paired Student's  t-test) in binding to AChE-treated solubilized compared to solubilized control samples.	bind
6304	2	2860	6	10	NULL	NULL	NULL	AChE	GP		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_133_7_1055_s_105	11487516	(A) Histogram showing the concentration curve for AChE enhancement of [3]-FW binding to AMPA receptors solubilized with 1% octylglucopyranoside There was a significant increase ( P<0.01, non paired Student's  t-test) in binding to AChE-treated solubilized compared to solubilized control samples.	bind
6149	1	2861	5	10	NULL	NULL	NULL	Gpa2p	GP		bind					GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_6110_s_284	10454558	(A) Histone H1 phosphorylation was assayed with GST-Ime2p purified from  E. coli and [gamma-32]ATP in the presence of BSA (lane 2), Gpa2p bound to GDP (lane 3), or Gpa2p bound to GTPgammaS (lane 4), washed free of unbound guanine nucleotides.	bind
6150	2	2861	5	10	NULL	NULL	NULL	Gpa2p	GP		bind					GTPgammaS	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_6110_s_284	10454558	(A) Histone H1 phosphorylation was assayed with GST-Ime2p purified from  E. coli and [gamma-32]ATP in the presence of BSA (lane 2), Gpa2p bound to GDP (lane 3), or Gpa2p bound to GTPgammaS (lane 4), washed free of unbound guanine nucleotides.	bind
6312	1	2861	6	10	NULL	NULL	NULL	Gpa2p	GP		bind					GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_6110_s_284	10454558	(A) Histone H1 phosphorylation was assayed with GST-Ime2p purified from  E. coli and [gamma-32]ATP in the presence of BSA (lane 2), Gpa2p bound to GDP (lane 3), or Gpa2p bound to GTPgammaS (lane 4), washed free of unbound guanine nucleotides.	bind
6314	2	2861	6	10	NULL	NULL	NULL	Gpa2p	GP		bind					GTPgammaS	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_6110_s_284	10454558	(A) Histone H1 phosphorylation was assayed with GST-Ime2p purified from  E. coli and [gamma-32]ATP in the presence of BSA (lane 2), Gpa2p bound to GDP (lane 3), or Gpa2p bound to GTPgammaS (lane 4), washed free of unbound guanine nucleotides.	bind
6151	1	2862	5	10	NULL	NULL	NULL	HMG-1	GP		bind					Z-3	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_186	10825199	(A) HMG-1 and ZEBRA bind cooperatively to Z-3 and Z-4.	bind
6152	2	2862	5	10	NULL	NULL	NULL	ZEBRA	GP		bind					Z-3	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_186	10825199	(A) HMG-1 and ZEBRA bind cooperatively to Z-3 and Z-4.	bind
6153	3	2862	5	10	NULL	NULL	NULL	statement 1	Process		occurs in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_186	10825199	(A) HMG-1 and ZEBRA bind cooperatively to Z-3 and Z-4.	bind
6154	4	2862	5	10	NULL	NULL	NULL	HMG-1	GP		bind					Z-4	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_186	10825199	(A) HMG-1 and ZEBRA bind cooperatively to Z-3 and Z-4.	bind
6155	5	2862	5	10	NULL	NULL	NULL	ZEBRA	GP		bind					Z-4	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_186	10825199	(A) HMG-1 and ZEBRA bind cooperatively to Z-3 and Z-4.	bind
6156	6	2862	5	10	NULL	NULL	NULL	statement 4	Process		occurs in cooperation with					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_186	10825199	(A) HMG-1 and ZEBRA bind cooperatively to Z-3 and Z-4.	bind
6417	1	2862	6	10	NULL	NULL	NULL	HMG-1	GP		bind					Z-3	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_186	10825199	(A) HMG-1 and ZEBRA bind cooperatively to Z-3 and Z-4.	bind
6418	2	2862	6	10	NULL	NULL	NULL	HMG-1	GP		bind					Z-4	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_186	10825199	(A) HMG-1 and ZEBRA bind cooperatively to Z-3 and Z-4.	bind
6419	3	2862	6	10	NULL	NULL	NULL	ZEBRA	GP		bind					Z-3	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_186	10825199	(A) HMG-1 and ZEBRA bind cooperatively to Z-3 and Z-4.	bind
6420	4	2862	6	10	NULL	NULL	NULL	ZEBRA	GP		bind					Z-4	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_186	10825199	(A) HMG-1 and ZEBRA bind cooperatively to Z-3 and Z-4.	bind
46525	5	2862	6	10	NULL	NULL	NULL	statement 1	Process		occurs in cooperation with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_186	10825199	(A) HMG-1 and ZEBRA bind cooperatively to Z-3 and Z-4.	bind
46526	6	2862	6	10	NULL	NULL	NULL	statement 2	Process		occurs in cooperation with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_186	10825199	(A) HMG-1 and ZEBRA bind cooperatively to Z-3 and Z-4.	bind
6157	2	2863	5	10	NULL	NULL	NULL	HSF	GP		bind					statement 1	Process				NULL	polytene chromosomes of wild-type larvae	NULL	NULL	NULL	NULL	gw70_cellbiol_161_4_707_s_127	12756231	(A) HSF and (B) POLII binding heat shock -  induced puffs in polytene chromosomes  of wild-type larvae.	bind
6158	3	2863	5	10	NULL	NULL	NULL	POLII	GP		bind					statement 1	Process				NULL	polytene chromosomes of wild-type larvae	NULL	NULL	NULL	NULL	gw70_cellbiol_161_4_707_s_127	12756231	(A) HSF and (B) POLII binding heat shock -  induced puffs in polytene chromosomes  of wild-type larvae.	bind
46527	1	2863	5	10	NULL	NULL	NULL	heat shock			induce					puffs	Chromosome				NULL	 polytene chromosomes of wild-type larvae	NULL	NULL	NULL	NULL	gw70_cellbiol_161_4_707_s_127	12756231	(A) HSF and (B) POLII binding heat shock -  induced puffs in polytene chromosomes  of wild-type larvae.	bind
6421	1	2863	6	10	NULL	NULL	NULL	heat shock			induces					puffs	Chromosome				NULL	in polytene chromosomes of wild-type larvae	NULL	NULL	NULL	NULL	gw70_cellbiol_161_4_707_s_127	12756231	(A) HSF and (B) POLII binding heat shock -  induced puffs in polytene chromosomes  of wild-type larvae.	bind
6422	2	2863	6	10	NULL	NULL	NULL	HSF	GP		bind					statement 1	Process				NULL	in polytene chromosomes of wild-type larvae	NULL	NULL	NULL	NULL	gw70_cellbiol_161_4_707_s_127	12756231	(A) HSF and (B) POLII binding heat shock -  induced puffs in polytene chromosomes  of wild-type larvae.	bind
6423	3	2863	6	10	NULL	NULL	NULL	POLII	GP		bind					statement 1	Process				NULL	in polytene chromosomes of wild-type larvae	NULL	NULL	NULL	NULL	gw70_cellbiol_161_4_707_s_127	12756231	(A) HSF and (B) POLII binding heat shock -  induced puffs in polytene chromosomes  of wild-type larvae.	bind
6159	1	2864	5	10	NULL	NULL	NULL	Hsp70	GP		bind					DC	Cell	human			NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_3_353_s_33	12354387	(A) Hsp70 binds to human DC by a mechanism with the characteristics of a saturable receptor system.	bind
6160	2	2864	5	10	NULL	NULL	NULL	statement 1	Process		involves					saturable receptor system	GP	mechanism of			NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_3_353_s_33	12354387	(A) Hsp70 binds to human DC by a mechanism with the characteristics of a saturable receptor system.	bind
6424	1	2864	6	10	NULL	NULL	NULL	Hsp70	GP		bind					DC	Cell	human			NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_3_353_s_33	12354387	(A) Hsp70 binds to human DC by a mechanism with the characteristics of a saturable receptor system.	bind
53071	2	2864	6	10	NULL	NULL	NULL	statement 1	Process		involves					 saturable receptor system	GP	mechanism of			NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_3_353_s_33	12354387	(A) Hsp70 binds to human DC by a mechanism with the characteristics of a saturable receptor system.	bind
6161	1	2865	5	10	NULL	NULL	NULL	hTR	GP		bind					hTERT	GP	mutant	E-region		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6234_s_200	12167716	(A) hTR binding to hTERT E-region mutants.	bind
6425	1	2865	6	10	NULL	NULL	NULL	hTR	GP		bind					hTERT	GP	mutant	E-region		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6234_s_200	12167716	(A) hTR binding to hTERT E-region mutants.	bind
6173	1	2869	5	10	NULL	NULL	NULL	MyoD	GP		bind		sequence specific			MEF-1 oligodeoxynucleotide	NucleicAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_307	11940648	(A) Id2, Id1, and Id3 inhibit the sequence-specific binding of MyoD to the MEF-1 oligodeoxynucleotide in vitro, and p204 overcomes the inhibition, as determined by EMSA.	bind
6174	2	2869	5	10	NULL	NULL	NULL	Id2	GP		inhibit					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_307	11940648	(A) Id2, Id1, and Id3 inhibit the sequence-specific binding of MyoD to the MEF-1 oligodeoxynucleotide in vitro, and p204 overcomes the inhibition, as determined by EMSA.	bind
6175	3	2869	5	10	NULL	NULL	NULL	Id1	GP		inhibit					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_307	11940648	(A) Id2, Id1, and Id3 inhibit the sequence-specific binding of MyoD to the MEF-1 oligodeoxynucleotide in vitro, and p204 overcomes the inhibition, as determined by EMSA.	bind
6176	4	2869	5	10	NULL	NULL	NULL	Id3	GP		inhibit					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_307	11940648	(A) Id2, Id1, and Id3 inhibit the sequence-specific binding of MyoD to the MEF-1 oligodeoxynucleotide in vitro, and p204 overcomes the inhibition, as determined by EMSA.	bind
6177	5	2869	5	10	NULL	NULL	NULL	p204	GP		overcomes					statement 2	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_307	11940648	(A) Id2, Id1, and Id3 inhibit the sequence-specific binding of MyoD to the MEF-1 oligodeoxynucleotide in vitro, and p204 overcomes the inhibition, as determined by EMSA.	bind
6178	6	2869	5	10	NULL	NULL	NULL	p204	GP		overcomes					statement 3	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_307	11940648	(A) Id2, Id1, and Id3 inhibit the sequence-specific binding of MyoD to the MEF-1 oligodeoxynucleotide in vitro, and p204 overcomes the inhibition, as determined by EMSA.	bind
6179	7	2869	5	10	NULL	NULL	NULL	p204	GP		overcomes					statement 4	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_307	11940648	(A) Id2, Id1, and Id3 inhibit the sequence-specific binding of MyoD to the MEF-1 oligodeoxynucleotide in vitro, and p204 overcomes the inhibition, as determined by EMSA.	bind
6432	1	2869	6	10	NULL	NULL	NULL	MyoD	GP		bind					MEF-1 oligodeoxynucleotide	NucleicAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_307	11940648	(A) Id2, Id1, and Id3 inhibit the sequence-specific binding of MyoD to the MEF-1 oligodeoxynucleotide in vitro, and p204 overcomes the inhibition, as determined by EMSA.	bind
6433	2	2869	6	10	NULL	NULL	NULL	Id1	GP		inhibit					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_307	11940648	(A) Id2, Id1, and Id3 inhibit the sequence-specific binding of MyoD to the MEF-1 oligodeoxynucleotide in vitro, and p204 overcomes the inhibition, as determined by EMSA.	bind
6434	3	2869	6	10	NULL	NULL	NULL	Id2	GP		inhibit					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_307	11940648	(A) Id2, Id1, and Id3 inhibit the sequence-specific binding of MyoD to the MEF-1 oligodeoxynucleotide in vitro, and p204 overcomes the inhibition, as determined by EMSA.	bind
6435	4	2869	6	10	NULL	NULL	NULL	Id3	GP		inhibit					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_307	11940648	(A) Id2, Id1, and Id3 inhibit the sequence-specific binding of MyoD to the MEF-1 oligodeoxynucleotide in vitro, and p204 overcomes the inhibition, as determined by EMSA.	bind
6436	5	2869	6	10	NULL	NULL	NULL	p204	GP		overcomes					statement 2	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_307	11940648	(A) Id2, Id1, and Id3 inhibit the sequence-specific binding of MyoD to the MEF-1 oligodeoxynucleotide in vitro, and p204 overcomes the inhibition, as determined by EMSA.	bind
6437	6	2869	6	10	NULL	NULL	NULL	p204	GP		overcomes					statement 3	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_307	11940648	(A) Id2, Id1, and Id3 inhibit the sequence-specific binding of MyoD to the MEF-1 oligodeoxynucleotide in vitro, and p204 overcomes the inhibition, as determined by EMSA.	bind
6438	7	2869	6	10	NULL	NULL	NULL	p204	GP		overcomes					statement 4	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_307	11940648	(A) Id2, Id1, and Id3 inhibit the sequence-specific binding of MyoD to the MEF-1 oligodeoxynucleotide in vitro, and p204 overcomes the inhibition, as determined by EMSA.	bind
6180	1	2870	5	10	NULL	NULL	NULL	IE2 protein	GP		does not bind					il1b	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_6803_s_328	10490619	(a) IE2 protein does not bind to the  il1b promoter.	bind
6439	1	2870	6	10	NULL	NULL	NULL	IE2 protein	GP		does not bind					il1b	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_6803_s_328	10490619	(a) IE2 protein does not bind to the  il1b promoter.	bind
6181	1	2872	5	10	NULL	NULL	NULL	preS2 peptide	AminoAcid		bind			120-132		r-HBsAg	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_febslett_441_3_407_s_144	9891981	(A) IgG and (B) scFv to r-HBsAg binding by preS2 peptides 120-132, 120-145 and 148-174.	bind
6182	2	2872	5	10	NULL	NULL	NULL	preS2 peptide	AminoAcid		bind			120-145		r-HBsAg	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_febslett_441_3_407_s_144	9891981	(A) IgG and (B) scFv to r-HBsAg binding by preS2 peptides 120-132, 120-145 and 148-174.	bind
6183	3	2872	5	10	NULL	NULL	NULL	preS2 peptide	AminoAcid		bind			148-174		r-HBsAg	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_febslett_441_3_407_s_144	9891981	(A) IgG and (B) scFv to r-HBsAg binding by preS2 peptides 120-132, 120-145 and 148-174.	bind
6962	1	2872	6	10	NULL	NULL	NULL	preS2 peptides	AminoAcid		bind			120-132		 r-HBsAg	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_febslett_441_3_407_s_144	9891981	(A) IgG and (B) scFv to r-HBsAg binding by preS2 peptides 120-132, 120-145 and 148-174.	bind
6963	2	2872	6	10	NULL	NULL	NULL	preS2 peptides 	AminoAcid		bind			120-145		 r-HBsAg	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_febslett_441_3_407_s_144	9891981	(A) IgG and (B) scFv to r-HBsAg binding by preS2 peptides 120-132, 120-145 and 148-174.	bind
46707	3	2872	6	10	NULL	NULL	NULL	preS2 peptides	AminoAcid		bind			148-174		r-HBsAg	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_febslett_441_3_407_s_144	9891981	(A) IgG and (B) scFv to r-HBsAg binding by preS2 peptides 120-132, 120-145 and 148-174.	bind
6184	1	2873	5	10	NULL	NULL	NULL	MT	CellComponent		bind					His6-CLASP2	GP	bacterially expressed	340 - 1084		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_169_6_929_s_184	15955847	(A) Immunoblot of a MT sedimentation assay of bacterially expressed His6-CLASP2(340  - 1084) at constant concentration incubated with increasing concentrations of MTs.  Note the slightly smaller degradation product ( 70 kD), which does not bind to MTs. (B) Comparison of MT binding of His6-CLASP2(340  - 1084) and His6-CLASP2(340 - 875).	bind
6185	2	2873	5	10	NULL	NULL	NULL	MT	CellComponent		bind					His6-CLASP2	GP	bacterially expressed	340 - 875		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_169_6_929_s_184	15955847	(A) Immunoblot of a MT sedimentation assay of bacterially expressed His6-CLASP2(340  - 1084) at constant concentration incubated with increasing concentrations of MTs.  Note the slightly smaller degradation product ( 70 kD), which does not bind to MTs. (B) Comparison of MT binding of His6-CLASP2(340  - 1084) and His6-CLASP2(340 - 875).	bind
6186	3	2873	5	10	NULL	NULL	NULL	70 kD degradation product	GP		does not bind					MT	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_169_6_929_s_184	15955847	(A) Immunoblot of a MT sedimentation assay of bacterially expressed His6-CLASP2(340  - 1084) at constant concentration incubated with increasing concentrations of MTs.  Note the slightly smaller degradation product ( 70 kD), which does not bind to MTs. (B) Comparison of MT binding of His6-CLASP2(340  - 1084) and His6-CLASP2(340 - 875).	bind
6440	1	2873	6	10	NULL	NULL	NULL	His6-CLASP2	GP	bacterially expressed	bind			340-1084		MT	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_169_6_929_s_184	15955847	(A) Immunoblot of a MT sedimentation assay of bacterially expressed His6-CLASP2(340  - 1084) at constant concentration incubated with increasing concentrations of MTs.  Note the slightly smaller degradation product ( 70 kD), which does not bind to MTs. (B) Comparison of MT binding of His6-CLASP2(340  - 1084) and His6-CLASP2(340 - 875).	bind
6441	2	2873	6	10	NULL	NULL	NULL	His6-CLASP2	GP	bacterially expressed	bind			340-875		MT	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_169_6_929_s_184	15955847	(A) Immunoblot of a MT sedimentation assay of bacterially expressed His6-CLASP2(340  - 1084) at constant concentration incubated with increasing concentrations of MTs.  Note the slightly smaller degradation product ( 70 kD), which does not bind to MTs. (B) Comparison of MT binding of His6-CLASP2(340  - 1084) and His6-CLASP2(340 - 875).	bind
46528	3	2873	6	10	NULL	NULL	NULL	70 kD degradation product	GP		does not bind					MT	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_169_6_929_s_184	15955847	(A) Immunoblot of a MT sedimentation assay of bacterially expressed His6-CLASP2(340  - 1084) at constant concentration incubated with increasing concentrations of MTs.  Note the slightly smaller degradation product ( 70 kD), which does not bind to MTs. (B) Comparison of MT binding of His6-CLASP2(340  - 1084) and His6-CLASP2(340 - 875).	bind
6187	1	2874	5	10	NULL	NULL	NULL	proteins	GP	rat brain deoxycholate extracts 	bind					microcystin-LR	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4690_s_234	12052877	(A) Immunoblots of proteins from rat brain deoxycholate extracts (input) bound to microcystin-LR-Sepharose.	bind
6442	1	2874	6	10	NULL	NULL	NULL	 protein	GP	rat brain deoxycholate extracts	bind					microcystin-LR	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4690_s_234	12052877	(A) Immunoblots of proteins from rat brain deoxycholate extracts (input) bound to microcystin-LR-Sepharose.	bind
6188	1	2875	5	10	NULL	NULL	NULL	Smad2	GP		bind					tubulin	GP				NULL	wild type Mv1Lu cells	NULL	NULL	NULL	NULL	gw60_molcell_5_1_27_s_51	10678166	(A) Immunoprecipitation of Mv1Lu cell lysates by an anti-tubulin antibody followed by Western blotting with a polyclonal anti-Smad2 antibody confirms the binding of Smad2 to tubulin in wild type and mutant Mv1Lu cells.	bind
6189	2	2875	5	10	NULL	NULL	NULL	Smad2	GP		bind					tubulin	GP				NULL	mutant Mv1Lu cells	NULL	NULL	NULL	NULL	gw60_molcell_5_1_27_s_51	10678166	(A) Immunoprecipitation of Mv1Lu cell lysates by an anti-tubulin antibody followed by Western blotting with a polyclonal anti-Smad2 antibody confirms the binding of Smad2 to tubulin in wild type and mutant Mv1Lu cells.	bind
6573	1	2875	6	10	NULL	NULL	NULL	Smad2	GP		bind					tubulin	GP				NULL	wild type Mv1Lu cells	NULL	NULL	NULL	NULL	gw60_molcell_5_1_27_s_51	10678166	(A) Immunoprecipitation of Mv1Lu cell lysates by an anti-tubulin antibody followed by Western blotting with a polyclonal anti-Smad2 antibody confirms the binding of Smad2 to tubulin in wild type and mutant Mv1Lu cells.	bind
6574	2	2875	6	10	NULL	NULL	NULL	Smad2	GP		bind					tubulin	GP				NULL	mutant Mv1Lu cells	NULL	NULL	NULL	NULL	gw60_molcell_5_1_27_s_51	10678166	(A) Immunoprecipitation of Mv1Lu cell lysates by an anti-tubulin antibody followed by Western blotting with a polyclonal anti-Smad2 antibody confirms the binding of Smad2 to tubulin in wild type and mutant Mv1Lu cells.	bind
6190	1	2878	5	10	NULL	NULL	NULL	Bcr	GP	constitutively active	phosphorylate					AF-6	GP				NULL	quiescent cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_13_4663_s_318	12808105	(A) In quiescent cells the constitutively active Bcr phosphorylates  AF-6 (step 1), which leads to the interaction of the PDZ domain of AF-6 with the  PDZ-binding motif of Bcr (step 2).	bind
6191	2	2878	5	10	NULL	NULL	NULL	AF-6	GP		bind			PDZ domain		Bcr	GP		PDZ-binding motif		NULL	quiescent cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_13_4663_s_318	12808105	(A) In quiescent cells the constitutively active Bcr phosphorylates  AF-6 (step 1), which leads to the interaction of the PDZ domain of AF-6 with the  PDZ-binding motif of Bcr (step 2).	bind
6192	3	2878	5	10	NULL	NULL	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_13_4663_s_318	12808105	(A) In quiescent cells the constitutively active Bcr phosphorylates  AF-6 (step 1), which leads to the interaction of the PDZ domain of AF-6 with the  PDZ-binding motif of Bcr (step 2).	bind
6577	1	2878	6	10	NULL	NULL	NULL	Bcr	GP	constitutively active	phosphorylates					AF-6	GP				NULL	quiescent cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_13_4663_s_318	12808105	(A) In quiescent cells the constitutively active Bcr phosphorylates  AF-6 (step 1), which leads to the interaction of the PDZ domain of AF-6 with the  PDZ-binding motif of Bcr (step 2).	bind
6580	2	2878	6	10	NULL	NULL	NULL	AF-6	GP		bind			PDZ domain		Bcr	GP		PDZ binding motif		NULL	quiescent cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_13_4663_s_318	12808105	(A) In quiescent cells the constitutively active Bcr phosphorylates  AF-6 (step 1), which leads to the interaction of the PDZ domain of AF-6 with the  PDZ-binding motif of Bcr (step 2).	bind
6581	3	2878	6	10	NULL	NULL	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_13_4663_s_318	12808105	(A) In quiescent cells the constitutively active Bcr phosphorylates  AF-6 (step 1), which leads to the interaction of the PDZ domain of AF-6 with the  PDZ-binding motif of Bcr (step 2).	bind
6193	1	2880	5	10	NULL	NULL	NULL	ephexin	GP		bind		stably			EphA receptors	GP				NULL	membrane	NULL	NULL	NULL	NULL	gw60_cell_105_2_233_s_270	11336673	(A) In regions of the growth cone  not in contact with ephrin-A, ephexin is stably  bound to EphA receptors at the membrane, where  ephexin contributes to the activation of RhoA, Cdc42, and  Rac1.	bind
6194	2	2880	5	10	NULL	NULL	NULL	ephexin	GP		contribute to					RhoA	GP	activation of			NULL	membrane	NULL	NULL	NULL	NULL	gw60_cell_105_2_233_s_270	11336673	(A) In regions of the growth cone  not in contact with ephrin-A, ephexin is stably  bound to EphA receptors at the membrane, where  ephexin contributes to the activation of RhoA, Cdc42, and  Rac1.	bind
6195	3	2880	5	10	NULL	NULL	NULL	ephexin	GP		contribute to					Cdc42	GP	activation of			NULL	membrane	NULL	NULL	NULL	NULL	gw60_cell_105_2_233_s_270	11336673	(A) In regions of the growth cone  not in contact with ephrin-A, ephexin is stably  bound to EphA receptors at the membrane, where  ephexin contributes to the activation of RhoA, Cdc42, and  Rac1.	bind
6196	4	2880	5	10	NULL	NULL	NULL	ephexin	GP		contribute to					Rac1	GP	activation of			NULL	membrane	NULL	NULL	NULL	NULL	gw60_cell_105_2_233_s_270	11336673	(A) In regions of the growth cone  not in contact with ephrin-A, ephexin is stably  bound to EphA receptors at the membrane, where  ephexin contributes to the activation of RhoA, Cdc42, and  Rac1.	bind
6583	1	2880	6	10	NULL	NULL	NULL	ephexin	GP		bind		stably			EphA receptors	GP				NULL	membrane	NULL	NULL	NULL	NULL	gw60_cell_105_2_233_s_270	11336673	(A) In regions of the growth cone  not in contact with ephrin-A, ephexin is stably  bound to EphA receptors at the membrane, where  ephexin contributes to the activation of RhoA, Cdc42, and  Rac1.	bind
6584	2	2880	6	10	NULL	NULL	NULL	ephexin	GP		contributes to					RhoA	GP	activation of			NULL	membrane	NULL	NULL	NULL	NULL	gw60_cell_105_2_233_s_270	11336673	(A) In regions of the growth cone  not in contact with ephrin-A, ephexin is stably  bound to EphA receptors at the membrane, where  ephexin contributes to the activation of RhoA, Cdc42, and  Rac1.	bind
6585	3	2880	6	10	NULL	NULL	NULL	ephexin	GP		contributes to					Cdc42	GP	activation of			NULL	membrane	NULL	NULL	NULL	NULL	gw60_cell_105_2_233_s_270	11336673	(A) In regions of the growth cone  not in contact with ephrin-A, ephexin is stably  bound to EphA receptors at the membrane, where  ephexin contributes to the activation of RhoA, Cdc42, and  Rac1.	bind
6588	4	2880	6	10	NULL	NULL	NULL	ephexin	GP		contributes to					Rac1	GP	activation of			NULL	membrane	NULL	NULL	NULL	NULL	gw60_cell_105_2_233_s_270	11336673	(A) In regions of the growth cone  not in contact with ephrin-A, ephexin is stably  bound to EphA receptors at the membrane, where  ephexin contributes to the activation of RhoA, Cdc42, and  Rac1.	bind
53072	1	2881	5	10	NULL	NULL	NULL				bind			Galpha subunit 		GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_4_3_495_s_33	15755912	(A) In the absence of an extracellular  ligand, the G protein is present as an inactive heterotrimer (Galpha is in green, Gbeta is in blue, and Ggamma is in red), with the Galpha subunit bound to GDP.	bind
53073	2	2881	5	10	NULL	NULL	NULL	G protein	GP		present as					heterotrimer		inactive			NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_4_3_495_s_33	15755912	(A) In the absence of an extracellular  ligand, the G protein is present as an inactive heterotrimer (Galpha is in green, Gbeta is in blue, and Ggamma is in red), with the Galpha subunit bound to GDP.	bind
53074	3	2881	5	10	NULL	NULL	NULL	statement 2	Process		in absence of					extracellular ligand	GP				NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_4_3_495_s_33	15755912	(A) In the absence of an extracellular  ligand, the G protein is present as an inactive heterotrimer (Galpha is in green, Gbeta is in blue, and Ggamma is in red), with the Galpha subunit bound to GDP.	bind
6590	1	2881	6	10	NULL	NULL	NULL				bind			Galpha subunit		GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_4_3_495_s_33	15755912	(A) In the absence of an extracellular  ligand, the G protein is present as an inactive heterotrimer (Galpha is in green, Gbeta is in blue, and Ggamma is in red), with the Galpha subunit bound to GDP.	bind
6593	2	2881	6	10	NULL	NULL	NULL	G protein	GP		present as an					heterotrimer		inactive			NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_4_3_495_s_33	15755912	(A) In the absence of an extracellular  ligand, the G protein is present as an inactive heterotrimer (Galpha is in green, Gbeta is in blue, and Ggamma is in red), with the Galpha subunit bound to GDP.	bind
6594	3	2881	6	10	NULL	NULL	NULL	statement 2	Process		occurs in absence of					extracellular ligand	GP				NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_4_3_495_s_33	15755912	(A) In the absence of an extracellular  ligand, the G protein is present as an inactive heterotrimer (Galpha is in green, Gbeta is in blue, and Ggamma is in red), with the Galpha subunit bound to GDP.	bind
6197	1	2882	5	10	NULL	NULL	NULL	CBP	GP		bind					CIITA	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_941_s_235	9858618	(A) In the absence of dexamethasone, CBP binds to CIITA.	bind
6198	2	2882	5	10	NULL	NULL	NULL	statement 1	Process		in the absence of					dexamethasone	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_941_s_235	9858618	(A) In the absence of dexamethasone, CBP binds to CIITA.	bind
6595	1	2882	6	10	NULL	NULL	NULL	CBP	GP		bind					CIITA	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_941_s_235	9858618	(A) In the absence of dexamethasone, CBP binds to CIITA.	bind
6596	2	2882	6	10	NULL	NULL	NULL	statement 1	Process		occurs in absence of					dexamethasone	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_941_s_235	9858618	(A) In the absence of dexamethasone, CBP binds to CIITA.	bind
6201	1	2883	5	10	NULL	NULL	NULL	Akt1	GP		bind					JIP1	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_35_4_697_s_278	12194869	(A) In the basal state, Akt1 binds JIP1, preventing formation of JIP1-mediated, proapoptotic JNK complexes.	bind
6202	2	2883	5	10	NULL	NULL	NULL	JIP1	GP		mediate					proapoptotic JNK complexes	GP	formation of			NULL		NULL	NULL	NULL	NULL	gw60_neuron_35_4_697_s_278	12194869	(A) In the basal state, Akt1 binds JIP1, preventing formation of JIP1-mediated, proapoptotic JNK complexes.	bind
6203	3	2883	5	10	NULL	NULL	NULL	statement 1	Process		prevent					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_35_4_697_s_278	12194869	(A) In the basal state, Akt1 binds JIP1, preventing formation of JIP1-mediated, proapoptotic JNK complexes.	bind
46529	4	2883	5	10	NULL	NULL	NULL	statement 1	Process		occurs in					basal state					NULL		NULL	NULL	NULL	NULL	gw60_neuron_35_4_697_s_278	12194869	(A) In the basal state, Akt1 binds JIP1, preventing formation of JIP1-mediated, proapoptotic JNK complexes.	bind
6598	1	2883	6	10	NULL	NULL	NULL	Akt1	GP		bind					JIP1	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_35_4_697_s_278	12194869	(A) In the basal state, Akt1 binds JIP1, preventing formation of JIP1-mediated, proapoptotic JNK complexes.	bind
6600	2	2883	6	10	NULL	NULL	NULL	statement 1	Process		occurs in the 					basal state					NULL		NULL	NULL	NULL	NULL	gw60_neuron_35_4_697_s_278	12194869	(A) In the basal state, Akt1 binds JIP1, preventing formation of JIP1-mediated, proapoptotic JNK complexes.	bind
6603	3	2883	6	10	NULL	NULL	NULL	JIP1	GP		mediates					proapoptotic JNK complexes	GP	formation of 			NULL		NULL	NULL	NULL	NULL	gw60_neuron_35_4_697_s_278	12194869	(A) In the basal state, Akt1 binds JIP1, preventing formation of JIP1-mediated, proapoptotic JNK complexes.	bind
6604	4	2883	6	10	NULL	NULL	NULL	statement 1	Process		prevents					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_35_4_697_s_278	12194869	(A) In the basal state, Akt1 binds JIP1, preventing formation of JIP1-mediated, proapoptotic JNK complexes.	bind
6199	1	2884	5	10	NULL	NULL	NULL	CPE	NucleicAcid		bind					CPEB	GP				NULL	oocyte cytoplasm	NULL	NULL	NULL	NULL	gw60_molcell_6_5_1253_s_137	11106762	(A) In the oocyte cytoplasm, the CPE is bound by CPEB even in unstimulated oocytes.	bind
6200	2	2884	5	10	NULL	NULL	NULL	CPE	NucleicAcid		bind					CPEB	GP				NULL	unstimulated oocytes	NULL	NULL	NULL	NULL	gw60_molcell_6_5_1253_s_137	11106762	(A) In the oocyte cytoplasm, the CPE is bound by CPEB even in unstimulated oocytes.	bind
6605	1	2884	6	10	NULL	NULL	NULL	CPE	NucleicAcid		bind					CPEB	GP				NULL	oocyte cytoplasm	NULL	NULL	NULL	NULL	gw60_molcell_6_5_1253_s_137	11106762	(A) In the oocyte cytoplasm, the CPE is bound by CPEB even in unstimulated oocytes.	bind
7278	2	2884	6	10	NULL	NULL	NULL	CPE	NucleicAcid		bind					CPEB	GP				NULL	unstimulated oocytes	NULL	NULL	NULL	NULL	gw60_molcell_6_5_1253_s_137	11106762	(A) In the oocyte cytoplasm, the CPE is bound by CPEB even in unstimulated oocytes.	bind
6267	1	2886	5	10	NULL	NULL	NULL	BLM	GP		bind					Top3alpha	GP				NULL	in PML nuclear bodies of unstressed cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_20_8925_s_310	16199871	(A) In unstressed cells, BLM is bound to Top3alpha in the PML nuclear bodies ( ) (bindings between two molecular species are shown as double-headed arrows.	bind
6611	1	2886	6	10	NULL	NULL	NULL	BLM	GP		bind					Top3alpha	GP				NULL	PML nuclear bodies in unstressed cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_20_8925_s_310	16199871	(A) In unstressed cells, BLM is bound to Top3alpha in the PML nuclear bodies ( ) (bindings between two molecular species are shown as double-headed arrows.	bind
53075	1	2887	5	10	NULL	NULL	NULL	pp F 	GP	In vitro - synthesized;;radiolabeled	bind					SecC	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_97_5_553_s_90	10367885	(A) In vitro - synthesized, radiolabeled pp F was bound to Sec complex (SecC) reconstituted into proteoliposomes  or incubated with liposomes lacking protein.	bind
53076	2	2887	5	10	NULL	NULL	NULL	SecC	GP		is					Sec complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_97_5_553_s_90	10367885	(A) In vitro - synthesized, radiolabeled pp F was bound to Sec complex (SecC) reconstituted into proteoliposomes  or incubated with liposomes lacking protein.	bind
53077	3	2887	5	10	NULL	NULL	NULL	SecC	GP		reconsituted into					proteoliposomes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cell_97_5_553_s_90	10367885	(A) In vitro - synthesized, radiolabeled pp F was bound to Sec complex (SecC) reconstituted into proteoliposomes  or incubated with liposomes lacking protein.	bind
6612	1	2887	6	10	NULL	NULL	NULL	pp F	GP	In vitro - synthesized;;radiolabeled	bind					SecC	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_97_5_553_s_90	10367885	(A) In vitro - synthesized, radiolabeled pp F was bound to Sec complex (SecC) reconstituted into proteoliposomes  or incubated with liposomes lacking protein.	bind
6613	2	2887	6	10	NULL	NULL	NULL	SecC	GP		is					Sec complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_97_5_553_s_90	10367885	(A) In vitro - synthesized, radiolabeled pp F was bound to Sec complex (SecC) reconstituted into proteoliposomes  or incubated with liposomes lacking protein.	bind
6615	3	2887	6	10	NULL	NULL	NULL	SecC	GP		reconstituted into					proteoliposomes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cell_97_5_553_s_90	10367885	(A) In vitro - synthesized, radiolabeled pp F was bound to Sec complex (SecC) reconstituted into proteoliposomes  or incubated with liposomes lacking protein.	bind
6269	1	2888	5	10	NULL	NULL	NULL	hADA3	GP		bind					p53	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_16_5801_s_205	12138191	(A) In vitro binding between hADA3 and p53.	bind
6621	1	2888	6	10	NULL	NULL	NULL	hADA3	GP		bind					p53	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_16_5801_s_205	12138191	(A) In vitro binding between hADA3 and p53.	bind
6270	1	2889	5	10	NULL	NULL	NULL	junD	GP		bind									A-TRE	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5073_s_107	9710591	(A) In vitro binding of  junD to the A-TRE is greatly enhanced in the presence of c- fos protein.	bind
6271	2	2889	5	10	NULL	NULL	NULL	statement 1	Process		enhance					c- fos protein	GP	in the presence of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5073_s_107	9710591	(A) In vitro binding of  junD to the A-TRE is greatly enhanced in the presence of c- fos protein.	bind
6622	1	2889	6	10	NULL	NULL	NULL	junD	GP		bind									A-TRE	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5073_s_107	9710591	(A) In vitro binding of  junD to the A-TRE is greatly enhanced in the presence of c- fos protein.	bind
6623	2	2889	6	10	NULL	NULL	NULL	statement 1	Process		enhanced					c-fos protein	GP	 in presence of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5073_s_107	9710591	(A) In vitro binding of  junD to the A-TRE is greatly enhanced in the presence of c- fos protein.	bind
6272	1	2890	5	10	NULL	NULL	NULL	CRM1s	GP		bind					RanBP3	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8751_s_251	14612415	(A) In vitro binding of CRM1s to RanBP3.	bind
6624	1	2890	6	10	NULL	NULL	NULL	CRM1s	GP		bind					RanBP3	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8751_s_251	14612415	(A) In vitro binding of CRM1s to RanBP3.	bind
6273	1	2891	5	10	NULL	NULL	NULL	GST-RhoA	GP		bind					GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_8_2650_s_240	11909959	(A) In vitro binding of Nir2 to GDP-bound GST-RhoA.	bind
6274	2	2891	5	10	NULL	NULL	NULL	Nir2	GP		bind					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_8_2650_s_240	11909959	(A) In vitro binding of Nir2 to GDP-bound GST-RhoA.	bind
6715	1	2891	6	10	NULL	NULL	NULL	GDP	Chemical		bind					GST-RhoA	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_8_2650_s_240	11909959	(A) In vitro binding of Nir2 to GDP-bound GST-RhoA.	bind
6716	2	2891	6	10	NULL	NULL	NULL	Nir2	GP		bind					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_8_2650_s_240	11909959	(A) In vitro binding of Nir2 to GDP-bound GST-RhoA.	bind
6275	1	2892	5	10	NULL	NULL	NULL	RB	GP		bind					GST-E2F-1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_4032_s_186	9632788	(A) In vitro binding of RB to GST-E2F-1.	bind
6717	1	2892	6	10	NULL	NULL	NULL	RB	GP		bind					GST-E2F-1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_4032_s_186	9632788	(A) In vitro binding of RB to GST-E2F-1.	bind
6718	1	2893	6	10	NULL	NULL	NULL	TBP	GP		bind					SNR6	GP			promoter	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6429_s_258	11533232	(A) In vitro binding of TBP to  SNR6 promoters.	bind
6277	1	2894	5	10	NULL	NULL	NULL	E2F1	GP		bind					p53	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_1_78_s_253	11739724	(A) In vitro competition assay using baculovirus-expressed cyclin A (2, 5, or 10 mug) to compete out the binding of E2F1 to p53.	bind
6278	2	2894	5	10	NULL	NULL	NULL	cyclin A	GP	baculovirus-expressed	bind					p53	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_1_78_s_253	11739724	(A) In vitro competition assay using baculovirus-expressed cyclin A (2, 5, or 10 mug) to compete out the binding of E2F1 to p53.	bind
6279	3	2894	5	10	NULL	NULL	NULL	statement 2	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_1_78_s_253	11739724	(A) In vitro competition assay using baculovirus-expressed cyclin A (2, 5, or 10 mug) to compete out the binding of E2F1 to p53.	bind
6719	1	2894	6	10	NULL	NULL	NULL	E2F1	GP		bind					p53	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_1_78_s_253	11739724	(A) In vitro competition assay using baculovirus-expressed cyclin A (2, 5, or 10 mug) to compete out the binding of E2F1 to p53.	bind
6720	2	2894	6	10	NULL	NULL	NULL	cyclin A	GP	baculovirus-expressed	bind					p53	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_1_78_s_253	11739724	(A) In vitro competition assay using baculovirus-expressed cyclin A (2, 5, or 10 mug) to compete out the binding of E2F1 to p53.	bind
6721	3	2894	6	10	NULL	NULL	NULL	statement 1	Process		competes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_1_78_s_253	11739724	(A) In vitro competition assay using baculovirus-expressed cyclin A (2, 5, or 10 mug) to compete out the binding of E2F1 to p53.	bind
6280	1	2895	5	10	NULL	NULL	NULL	Stat1-ER chimera	GP		bind					DNA	NucleicAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_2913_s_151	10082558	(A) In vitro DNA binding of the Stat1-ER chimera.	bind
6722	1	2895	6	10	NULL	NULL	NULL	DNA	NucleicAcid		bind					Stat1-ER chimera	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_2913_s_151	10082558	(A) In vitro DNA binding of the Stat1-ER chimera.	bind
7104	1	2900	5	10	NULL	NULL	NULL	MEF2 protein	GP	in vitro-translated	bind					Act57B	GP			MEF2 site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_mechdev_110_1_39_s_153	11744367	(A) In vitro translated MEF2 protein bound to the MEF2 site (complex b), is competed with a wild type MEF2 oligonucleotide sequence (wtMEF2), and is competed only weakly by a mutant MEF2 oligonucleotide sequence (mMEF2), demonstrating specificity for MEF2 binding within the context of the  Act57B promoter.	bind
7105	2	2900	5	10	NULL	NULL	NULL	wtMEF2	NucleicAcid		bind					Act57B	GP			MEF2 site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_mechdev_110_1_39_s_153	11744367	(A) In vitro translated MEF2 protein bound to the MEF2 site (complex b), is competed with a wild type MEF2 oligonucleotide sequence (wtMEF2), and is competed only weakly by a mutant MEF2 oligonucleotide sequence (mMEF2), demonstrating specificity for MEF2 binding within the context of the  Act57B promoter.	bind
7106	4	2900	5	10	NULL	NULL	NULL	statement 1	Process		compete with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_110_1_39_s_153	11744367	(A) In vitro translated MEF2 protein bound to the MEF2 site (complex b), is competed with a wild type MEF2 oligonucleotide sequence (wtMEF2), and is competed only weakly by a mutant MEF2 oligonucleotide sequence (mMEF2), demonstrating specificity for MEF2 binding within the context of the  Act57B promoter.	bind
7107	5	2900	5	10	NULL	NULL	NULL	mMEF2	NucleicAcid		bind		weakly			Act57B	GP			MEF2 site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_mechdev_110_1_39_s_153	11744367	(A) In vitro translated MEF2 protein bound to the MEF2 site (complex b), is competed with a wild type MEF2 oligonucleotide sequence (wtMEF2), and is competed only weakly by a mutant MEF2 oligonucleotide sequence (mMEF2), demonstrating specificity for MEF2 binding within the context of the  Act57B promoter.	bind
7108	6	2900	5	10	NULL	NULL	NULL	mMEF2	NucleicAcid		is					mutant MEF2 oligonucleotide sequence 	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_110_1_39_s_153	11744367	(A) In vitro translated MEF2 protein bound to the MEF2 site (complex b), is competed with a wild type MEF2 oligonucleotide sequence (wtMEF2), and is competed only weakly by a mutant MEF2 oligonucleotide sequence (mMEF2), demonstrating specificity for MEF2 binding within the context of the  Act57B promoter.	bind
7109	3	2900	5	10	NULL	NULL	NULL	wtMEF2	NucleicAcid		is					wild type MEF2 oligonucleotide sequence 	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_110_1_39_s_153	11744367	(A) In vitro translated MEF2 protein bound to the MEF2 site (complex b), is competed with a wild type MEF2 oligonucleotide sequence (wtMEF2), and is competed only weakly by a mutant MEF2 oligonucleotide sequence (mMEF2), demonstrating specificity for MEF2 binding within the context of the  Act57B promoter.	bind
7111	7	2900	5	10	NULL	NULL	NULL	statement 1	Process		compete with		weakly			statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_110_1_39_s_153	11744367	(A) In vitro translated MEF2 protein bound to the MEF2 site (complex b), is competed with a wild type MEF2 oligonucleotide sequence (wtMEF2), and is competed only weakly by a mutant MEF2 oligonucleotide sequence (mMEF2), demonstrating specificity for MEF2 binding within the context of the  Act57B promoter.	bind
6723	1	2900	6	10	NULL	NULL	NULL	MEF2 protein	GP	in vitro-translated	bind					Act57B 	GP			MEF2 site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_mechdev_110_1_39_s_153	11744367	(A) In vitro translated MEF2 protein bound to the MEF2 site (complex b), is competed with a wild type MEF2 oligonucleotide sequence (wtMEF2), and is competed only weakly by a mutant MEF2 oligonucleotide sequence (mMEF2), demonstrating specificity for MEF2 binding within the context of the  Act57B promoter.	bind
6724	2	2900	6	10	NULL	NULL	NULL	MEF2 oligoucleotide	NucleicAcid	wild type	bind					Act57B 	GP			MEF2 site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_mechdev_110_1_39_s_153	11744367	(A) In vitro translated MEF2 protein bound to the MEF2 site (complex b), is competed with a wild type MEF2 oligonucleotide sequence (wtMEF2), and is competed only weakly by a mutant MEF2 oligonucleotide sequence (mMEF2), demonstrating specificity for MEF2 binding within the context of the  Act57B promoter.	bind
6725	3	2900	6	10	NULL	NULL	NULL	statement 1	Process		competes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_110_1_39_s_153	11744367	(A) In vitro translated MEF2 protein bound to the MEF2 site (complex b), is competed with a wild type MEF2 oligonucleotide sequence (wtMEF2), and is competed only weakly by a mutant MEF2 oligonucleotide sequence (mMEF2), demonstrating specificity for MEF2 binding within the context of the  Act57B promoter.	bind
6726	4	2900	6	10	NULL	NULL	NULL	MEF2 oligoucleotide	NucleicAcid	mutant	bind		weakly			Act57B 	GP			MEF2 site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_mechdev_110_1_39_s_153	11744367	(A) In vitro translated MEF2 protein bound to the MEF2 site (complex b), is competed with a wild type MEF2 oligonucleotide sequence (wtMEF2), and is competed only weakly by a mutant MEF2 oligonucleotide sequence (mMEF2), demonstrating specificity for MEF2 binding within the context of the  Act57B promoter.	bind
6727	5	2900	6	10	NULL	NULL	NULL	statement 1	Process		competes		weakly			statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_110_1_39_s_153	11744367	(A) In vitro translated MEF2 protein bound to the MEF2 site (complex b), is competed with a wild type MEF2 oligonucleotide sequence (wtMEF2), and is competed only weakly by a mutant MEF2 oligonucleotide sequence (mMEF2), demonstrating specificity for MEF2 binding within the context of the  Act57B promoter.	bind
53078	6	2900	6	10	NULL	NULL	NULL	wtMEF2	NucleicAcid		is					wild type MEF2 oligonucleotide sequence 	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_110_1_39_s_153	11744367	(A) In vitro translated MEF2 protein bound to the MEF2 site (complex b), is competed with a wild type MEF2 oligonucleotide sequence (wtMEF2), and is competed only weakly by a mutant MEF2 oligonucleotide sequence (mMEF2), demonstrating specificity for MEF2 binding within the context of the  Act57B promoter.	bind
53079	7	2900	6	10	NULL	NULL	NULL	mMEF2	NucleicAcid		is					mutant MEF2 oligonucleotide sequence 	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_110_1_39_s_153	11744367	(A) In vitro translated MEF2 protein bound to the MEF2 site (complex b), is competed with a wild type MEF2 oligonucleotide sequence (wtMEF2), and is competed only weakly by a mutant MEF2 oligonucleotide sequence (mMEF2), demonstrating specificity for MEF2 binding within the context of the  Act57B promoter.	bind
6285	1	2901	5	10	NULL	NULL	NULL	Hrs	GP	in vitro translated;;35S-labeled	bind					GST-RGS-PX1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_12_5538_s_140	15469987	(A) In vitro translated, 35S-labeled Hrs binds to GST-RGS-PX1(PXC) but not to GST alone.	bind
6286	2	2901	5	10	NULL	NULL	NULL	Hrs	GP	in vitro-translated;;35S labeled	does not bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_12_5538_s_140	15469987	(A) In vitro translated, 35S-labeled Hrs binds to GST-RGS-PX1(PXC) but not to GST alone.	bind
6728	1	2901	6	10	NULL	NULL	NULL	Hrs	GP	in vitro-translated;;35S labeled	bind					GST-RGS-PX1	GP			PXC	NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_12_5538_s_140	15469987	(A) In vitro translated, 35S-labeled Hrs binds to GST-RGS-PX1(PXC) but not to GST alone.	bind
6729	2	2901	6	10	NULL	NULL	NULL	Hrs	GP	in vitro-translated;;35S labeled	does not bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_12_5538_s_140	15469987	(A) In vitro translated, 35S-labeled Hrs binds to GST-RGS-PX1(PXC) but not to GST alone.	bind
6287	1	2902	5	10	NULL	NULL	NULL	Ada	GP		is					Adaptin	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_2_221_s_158	12194853	(A) In vitro-translated  -Adaptin (Ada) protein binds GST-Numb, but not GST.	bind
6288	2	2902	5	10	NULL	NULL	NULL	Ada protein	GP	in vitro-translated	bind					GST-Numb	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_2_221_s_158	12194853	(A) In vitro-translated  -Adaptin (Ada) protein binds GST-Numb, but not GST.	bind
6289	3	2902	5	10	NULL	NULL	NULL	Ada protein	GP	in vitro translated	does not bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_2_221_s_158	12194853	(A) In vitro-translated  -Adaptin (Ada) protein binds GST-Numb, but not GST.	bind
6730	1	2902	6	10	NULL	NULL	NULL	Adaptin	GP	in vitro-translated	bind					GST-Numb	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_2_221_s_158	12194853	(A) In vitro-translated  -Adaptin (Ada) protein binds GST-Numb, but not GST.	bind
6731	2	2902	6	10	NULL	NULL	NULL	Adaptin	GP	in vitro-translated	does not bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_2_221_s_158	12194853	(A) In vitro-translated  -Adaptin (Ada) protein binds GST-Numb, but not GST.	bind
6732	3	2902	6	10	NULL	NULL	NULL	Adaptin	GP		is					Ada	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_2_221_s_158	12194853	(A) In vitro-translated  -Adaptin (Ada) protein binds GST-Numb, but not GST.	bind
6290	1	2903	5	10	NULL	0	NULL	ARVCF	NULL	in vitro-translated	bind	NULL				ZO-1	NULL		PDZ domains		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_12_5503_s_103	15456900	(A) In vitro-translated ARVCF binds to a GST fusion protein  containing the PDZ domains of ZO-1.	bind
46547	2	2903	5	10	NULL	0	NULL	ZO-1	NULL		is a type of	NULL		PDZ domain		 GST fusion protein 	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_12_5503_s_103	15456900	(A) In vitro-translated ARVCF binds to a GST fusion protein  containing the PDZ domains of ZO-1.	bind
6733	1	2903	6	10	NULL	0	NULL	ARVCF	NULL	in vitro-translated	bind	NULL				ZO-1	NULL		PDZ domain		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_12_5503_s_103	15456900	(A) In vitro-translated ARVCF binds to a GST fusion protein  containing the PDZ domains of ZO-1.	bind
46548	2	2903	6	10	NULL	0	NULL	ZO-1	NULL		is a type of	NULL		PDZ domain		GST fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_12_5503_s_103	15456900	(A) In vitro-translated ARVCF binds to a GST fusion protein  containing the PDZ domains of ZO-1.	bind
6292	1	2904	5	10	NULL	NULL	NULL	p150Glued	GP	in vitro-translated;; full length	bind					GST-EB1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_4_1405_s_122	12686597	(A) In vitro-translated full-length p150Glued was retained on a GST-EB1 column, but amino-terminal p150Glued deletion constructs p135MMRQ, pMT7-1, and pMT1-1 did not bind significantly to GST-EB1.	bind
6293	2	2904	5	10	NULL	NULL	NULL	p135MMRQ	AminoAcid		is a type of					p150Glued 	GP	deletion construct	amino-terminal 		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_4_1405_s_122	12686597	(A) In vitro-translated full-length p150Glued was retained on a GST-EB1 column, but amino-terminal p150Glued deletion constructs p135MMRQ, pMT7-1, and pMT1-1 did not bind significantly to GST-EB1.	bind
6294	3	2904	5	10	NULL	NULL	NULL	pMT7-1	AminoAcid		is a type of					p150Glued 	GP	deletion construct	amino-terminal		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_4_1405_s_122	12686597	(A) In vitro-translated full-length p150Glued was retained on a GST-EB1 column, but amino-terminal p150Glued deletion constructs p135MMRQ, pMT7-1, and pMT1-1 did not bind significantly to GST-EB1.	bind
6295	4	2904	5	10	NULL	NULL	NULL	pMT1-1	AminoAcid		is a type of					p150Glued 	GP	deletion construct	amino-terminal		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_4_1405_s_122	12686597	(A) In vitro-translated full-length p150Glued was retained on a GST-EB1 column, but amino-terminal p150Glued deletion constructs p135MMRQ, pMT7-1, and pMT1-1 did not bind significantly to GST-EB1.	bind
6296	5	2904	5	10	NULL	NULL	NULL	statement 2	AminoAcid		does not bind		significantly			GST-EB1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_4_1405_s_122	12686597	(A) In vitro-translated full-length p150Glued was retained on a GST-EB1 column, but amino-terminal p150Glued deletion constructs p135MMRQ, pMT7-1, and pMT1-1 did not bind significantly to GST-EB1.	bind
6297	6	2904	5	10	NULL	NULL	NULL	statement 3	AminoAcid		does not bind		significantly			GST-EB1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_4_1405_s_122	12686597	(A) In vitro-translated full-length p150Glued was retained on a GST-EB1 column, but amino-terminal p150Glued deletion constructs p135MMRQ, pMT7-1, and pMT1-1 did not bind significantly to GST-EB1.	bind
6298	7	2904	5	10	NULL	NULL	NULL	statement 4	AminoAcid		does not bind		significantly			GST-EB1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_4_1405_s_122	12686597	(A) In vitro-translated full-length p150Glued was retained on a GST-EB1 column, but amino-terminal p150Glued deletion constructs p135MMRQ, pMT7-1, and pMT1-1 did not bind significantly to GST-EB1.	bind
6734	1	2904	6	10	NULL	NULL	NULL	p150Glued	GP	in vitro-translated;;full length	bind					GST-EB1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_4_1405_s_122	12686597	(A) In vitro-translated full-length p150Glued was retained on a GST-EB1 column, but amino-terminal p150Glued deletion constructs p135MMRQ, pMT7-1, and pMT1-1 did not bind significantly to GST-EB1.	bind
6735	2	2904	6	10	NULL	NULL	NULL	p135MMRQ	AminoAcid		is a type of					 p150Glued	GP	deletion construct	amino-terminal		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_4_1405_s_122	12686597	(A) In vitro-translated full-length p150Glued was retained on a GST-EB1 column, but amino-terminal p150Glued deletion constructs p135MMRQ, pMT7-1, and pMT1-1 did not bind significantly to GST-EB1.	bind
6736	3	2904	6	10	NULL	NULL	NULL	pMT7-1	AminoAcid		is a type of					p150Glued	GP	deletion construct	amino-terminal		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_4_1405_s_122	12686597	(A) In vitro-translated full-length p150Glued was retained on a GST-EB1 column, but amino-terminal p150Glued deletion constructs p135MMRQ, pMT7-1, and pMT1-1 did not bind significantly to GST-EB1.	bind
6737	4	2904	6	10	NULL	NULL	NULL	pMT1-1	AminoAcid		is a type of					p150Glued	GP	deletion construct	amino-terminal		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_4_1405_s_122	12686597	(A) In vitro-translated full-length p150Glued was retained on a GST-EB1 column, but amino-terminal p150Glued deletion constructs p135MMRQ, pMT7-1, and pMT1-1 did not bind significantly to GST-EB1.	bind
53110	5	2904	6	10	NULL	NULL	NULL	statement 2	AminoAcid		does not bind		significantly			GST-EB1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_4_1405_s_122	12686597	(A) In vitro-translated full-length p150Glued was retained on a GST-EB1 column, but amino-terminal p150Glued deletion constructs p135MMRQ, pMT7-1, and pMT1-1 did not bind significantly to GST-EB1.	bind
53111	6	2904	6	10	NULL	NULL	NULL	statement 3	AminoAcid		does not bind		significantly			GST-EB1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_4_1405_s_122	12686597	(A) In vitro-translated full-length p150Glued was retained on a GST-EB1 column, but amino-terminal p150Glued deletion constructs p135MMRQ, pMT7-1, and pMT1-1 did not bind significantly to GST-EB1.	bind
53112	7	2904	6	10	NULL	NULL	NULL	statement 4	AminoAcid		does not bind		significantly			GST-EB1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_4_1405_s_122	12686597	(A) In vitro-translated full-length p150Glued was retained on a GST-EB1 column, but amino-terminal p150Glued deletion constructs p135MMRQ, pMT7-1, and pMT1-1 did not bind significantly to GST-EB1.	bind
6299	1	2905	5	10	NULL	NULL	NULL	Galphas	GP	in vitro translated;;35S-labeled	bind					GST-Hrs	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_12_5538_s_156	15469987	(A) In vitro-translated, 35S-labeled Galphas binds to GST-Hrs but not to GST alone.	bind
6301	2	2905	5	10	NULL	NULL	NULL	Galphas	GP	in vitro translated;;35S-labeled	does not bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_12_5538_s_156	15469987	(A) In vitro-translated, 35S-labeled Galphas binds to GST-Hrs but not to GST alone.	bind
6738	1	2905	6	10	NULL	NULL	NULL	Galphas	GP	in vitro-translated;;35S labeled	bind					GST-Hrs	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_12_5538_s_156	15469987	(A) In vitro-translated, 35S-labeled Galphas binds to GST-Hrs but not to GST alone.	bind
6739	2	2905	6	10	NULL	NULL	NULL	Galphas	GP	in vitro-translated;;35S labeled	does not bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_12_5538_s_156	15469987	(A) In vitro-translated, 35S-labeled Galphas binds to GST-Hrs but not to GST alone.	bind
6305	1	2906	5	10	NULL	NULL	NULL	IRF-5	GP		bind					IFNA	GP	endogenous		promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_16_5721_s_390	12138184	(A) In vivo binding of IRF-5 and IRF-3 to the endogenous IFNA promoter as analyzed by the chromatin immunoprecipitation assay.	bind
6306	2	2906	5	10	NULL	NULL	NULL	IRF-3	GP		bind					IFNA	GP	endogenous		promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_16_5721_s_390	12138184	(A) In vivo binding of IRF-5 and IRF-3 to the endogenous IFNA promoter as analyzed by the chromatin immunoprecipitation assay.	bind
6740	1	2906	6	10	NULL	NULL	NULL	IRF-5	GP		bind					IFNA	GP	endogenous		promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_16_5721_s_390	12138184	(A) In vivo binding of IRF-5 and IRF-3 to the endogenous IFNA promoter as analyzed by the chromatin immunoprecipitation assay.	bind
6741	2	2906	6	10	NULL	NULL	NULL	IRF-3	GP		bind					IFNA	GP	endogenous		promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_16_5721_s_390	12138184	(A) In vivo binding of IRF-5 and IRF-3 to the endogenous IFNA promoter as analyzed by the chromatin immunoprecipitation assay.	bind
7116	1	2907	5	10	NULL	NULL	NULL	PI(4)P shuttle	GP		bind					AP-1	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_cell_114_3_299_s_164	12914695	(A) In vivo rescue of  -adaptin (AP-1) binding by shuttle PI(4)P. PI4KII  RNAi cells were incubated with polyamine shuttle carriers in the presence or absence of 20  M diC16-PI(4)P or diC16-PIP2 for 30 min at 37 degrees C.	bind
7117	2	2907	5	10	NULL	NULL	NULL	AP-1	GP		is					adaptin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_3_299_s_164	12914695	(A) In vivo rescue of  -adaptin (AP-1) binding by shuttle PI(4)P. PI4KII  RNAi cells were incubated with polyamine shuttle carriers in the presence or absence of 20  M diC16-PI(4)P or diC16-PIP2 for 30 min at 37 degrees C.	bind
6742	1	2907	6	10	NULL	NULL	NULL	adaptin	GP		bind					shuttle PI(4)P	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_cell_114_3_299_s_164	12914695	(A) In vivo rescue of  -adaptin (AP-1) binding by shuttle PI(4)P. PI4KII  RNAi cells were incubated with polyamine shuttle carriers in the presence or absence of 20  M diC16-PI(4)P or diC16-PIP2 for 30 min at 37 degrees C.	bind
46549	2	2907	6	10	NULL	NULL	NULL	AP-1	GP		is					adaptin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_3_299_s_164	12914695	(A) In vivo rescue of  -adaptin (AP-1) binding by shuttle PI(4)P. PI4KII  RNAi cells were incubated with polyamine shuttle carriers in the presence or absence of 20  M diC16-PI(4)P or diC16-PIP2 for 30 min at 37 degrees C.	bind
6307	1	2908	5	10	NULL	NULL	NULL	Sir3	GP		bind					Sir4	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_11_4514_s_385	15899856	(A) In wild-type cells, the nucleation  and spreading of silent chromatin require both the binding of Sir3 to Sir4 and the  deacetylation of nucleosomes by Sir2.	bind
6308	2	2908	5	10	NULL	NULL	NULL	Sir2	GP		deacetylate					nucleosomes	Chromosome				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_11_4514_s_385	15899856	(A) In wild-type cells, the nucleation  and spreading of silent chromatin require both the binding of Sir3 to Sir4 and the  deacetylation of nucleosomes by Sir2.	bind
6392	3	2908	5	10	NULL	NULL	NULL	silent chromatin	Chromosome	nucleation of 	require					statement 1	Process				NULL	wild-type cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_11_4514_s_385	15899856	(A) In wild-type cells, the nucleation  and spreading of silent chromatin require both the binding of Sir3 to Sir4 and the  deacetylation of nucleosomes by Sir2.	bind
6393	4	2908	5	10	NULL	NULL	NULL	silent chromatin	Chromosome	nucleation of	require					statement 2	Process				NULL	wild-type cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_11_4514_s_385	15899856	(A) In wild-type cells, the nucleation  and spreading of silent chromatin require both the binding of Sir3 to Sir4 and the  deacetylation of nucleosomes by Sir2.	bind
6394	5	2908	5	10	NULL	0	NULL	silent chromatin	NULL	spreading of 	require	NULL				statement 1	NULL				NULL	wild-type cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_11_4514_s_385	15899856	(A) In wild-type cells, the nucleation  and spreading of silent chromatin require both the binding of Sir3 to Sir4 and the  deacetylation of nucleosomes by Sir2.	bind
6395	6	2908	5	10	NULL	NULL	NULL	silent chromatin	Chromosome	spreading of	require					statement 2	Process				NULL	wild-type cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_11_4514_s_385	15899856	(A) In wild-type cells, the nucleation  and spreading of silent chromatin require both the binding of Sir3 to Sir4 and the  deacetylation of nucleosomes by Sir2.	bind
6743	1	2908	6	10	NULL	NULL	NULL	Sir3	GP		bind					Sir4	GP				NULL	wild type cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_11_4514_s_385	15899856	(A) In wild-type cells, the nucleation  and spreading of silent chromatin require both the binding of Sir3 to Sir4 and the  deacetylation of nucleosomes by Sir2.	bind
6744	2	2908	6	10	NULL	NULL	NULL	Sir2	GP		deacetylates					nucleosomes	Chromosome				NULL	wild type cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_11_4514_s_385	15899856	(A) In wild-type cells, the nucleation  and spreading of silent chromatin require both the binding of Sir3 to Sir4 and the  deacetylation of nucleosomes by Sir2.	bind
6745	3	2908	6	10	NULL	NULL	NULL	silent chromatin	Chromosome	nucleation  of	require					statement 1	Process				NULL	wild type cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_11_4514_s_385	15899856	(A) In wild-type cells, the nucleation  and spreading of silent chromatin require both the binding of Sir3 to Sir4 and the  deacetylation of nucleosomes by Sir2.	bind
6746	4	2908	6	10	NULL	NULL	NULL	silent chromatin	Chromosome	nucleation of	require					statement 2	Process				NULL	wild type cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_11_4514_s_385	15899856	(A) In wild-type cells, the nucleation  and spreading of silent chromatin require both the binding of Sir3 to Sir4 and the  deacetylation of nucleosomes by Sir2.	bind
46556	5	2908	6	10	NULL	NULL	NULL	silent chromatin	Chromosome	spreading of	require					statement 1	Process				NULL	wild-type cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_11_4514_s_385	15899856	(A) In wild-type cells, the nucleation  and spreading of silent chromatin require both the binding of Sir3 to Sir4 and the  deacetylation of nucleosomes by Sir2.	bind
46557	6	2908	6	10	NULL	NULL	NULL	silent chromatin	Chromosome	spreading of	require					statement 2	Process				NULL	wild-type cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_11_4514_s_385	15899856	(A) In wild-type cells, the nucleation  and spreading of silent chromatin require both the binding of Sir3 to Sir4 and the  deacetylation of nucleosomes by Sir2.	bind
6396	1	2909	5	10	NULL	NULL	NULL	NEM	Chemical		inactivate					UBE	NucleicAcid	binding activity of			NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_72_1_65_s_129	10521600	(A) Inactivation of the UBE binding activity by NEM.	bind
6747	1	2909	6	10	NULL	NULL	NULL	NEM	Chemical		inactivates					UBE	NucleicAcid	binding activity of 			NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_72_1_65_s_129	10521600	(A) Inactivation of the UBE binding activity by NEM.	bind
6397	1	2911	5	10	NULL	NULL	NULL	Pex14p ligand	GP		bind					Pex13p	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_5_1007_s_106	12453410	(A) Independent binding of the Pex14p and Pex5p ligands to the Pex13p SH3 domain.	bind
6398	2	2911	5	10	NULL	NULL	NULL	Pex5p ligand	GP		bind					Pex13p	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_5_1007_s_106	12453410	(A) Independent binding of the Pex14p and Pex5p ligands to the Pex13p SH3 domain.	bind
6399	3	2911	5	10	NULL	NULL	NULL	statement 1	Process		is independent of					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_5_1007_s_106	12453410	(A) Independent binding of the Pex14p and Pex5p ligands to the Pex13p SH3 domain.	bind
6798	1	2911	6	10	NULL	NULL	NULL	Pex14p	GP		bind					Pex13p	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_5_1007_s_106	12453410	(A) Independent binding of the Pex14p and Pex5p ligands to the Pex13p SH3 domain.	bind
6799	2	2911	6	10	NULL	NULL	NULL	Pex5p	GP		bind					Pex13p	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_5_1007_s_106	12453410	(A) Independent binding of the Pex14p and Pex5p ligands to the Pex13p SH3 domain.	bind
7875	3	2911	6	10	NULL	NULL	NULL	statement 1	Process		is independent of					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_5_1007_s_106	12453410	(A) Independent binding of the Pex14p and Pex5p ligands to the Pex13p SH3 domain.	bind
6400	1	2912	5	10	NULL	NULL	NULL	Sp1	GP		bind					DNA	NucleicAcid				NULL	Hep3B cells	NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_4_1005_s_110	12200149	(A) Induction of the DNA-binding activity of Sp1 by TSA treatment in Hep3B cells.	bind
6401	2	2912	5	10	NULL	NULL	NULL	TSA	Chemical		induce					statement 1	Process				NULL	Hep3B cells	NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_4_1005_s_110	12200149	(A) Induction of the DNA-binding activity of Sp1 by TSA treatment in Hep3B cells.	bind
6800	1	2912	6	10	NULL	NULL	NULL	Sp1	GP		bind					DNA	NucleicAcid				NULL	Hep3B cells	NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_4_1005_s_110	12200149	(A) Induction of the DNA-binding activity of Sp1 by TSA treatment in Hep3B cells.	bind
6801	2	2912	6	10	NULL	NULL	NULL	TSA	Chemical		induces					statement 1	Process				NULL	Hep3B cells	NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_4_1005_s_110	12200149	(A) Induction of the DNA-binding activity of Sp1 by TSA treatment in Hep3B cells.	bind
6402	1	2913	5	10	NULL	NULL	NULL	ALDO	GP		bind					MR	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1589_1_31_s_140	11909639	(A) Inhibition of ALDO binding to MR by PLP is concentration- and time-dependent.	bind
6403	2	2913	5	10	NULL	NULL	NULL	PLP	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1589_1_31_s_140	11909639	(A) Inhibition of ALDO binding to MR by PLP is concentration- and time-dependent.	bind
6404	3	2913	5	10	NULL	NULL	NULL	statement 2	Process		is dependent on					concentration	QuantityOrMeasure				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1589_1_31_s_140	11909639	(A) Inhibition of ALDO binding to MR by PLP is concentration- and time-dependent.	bind
6405	4	2913	5	10	NULL	NULL	NULL	statement 2	Process		is dependent on					time	Time				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1589_1_31_s_140	11909639	(A) Inhibition of ALDO binding to MR by PLP is concentration- and time-dependent.	bind
6802	1	2913	6	10	NULL	NULL	NULL	ALDO	GP		bind					MR	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1589_1_31_s_140	11909639	(A) Inhibition of ALDO binding to MR by PLP is concentration- and time-dependent.	bind
6803	2	2913	6	10	NULL	NULL	NULL	PLP	Chemical		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1589_1_31_s_140	11909639	(A) Inhibition of ALDO binding to MR by PLP is concentration- and time-dependent.	bind
6804	3	2913	6	10	NULL	NULL	NULL	statement 2	Process		is dependent on					concentration	QuantityOrMeasure				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1589_1_31_s_140	11909639	(A) Inhibition of ALDO binding to MR by PLP is concentration- and time-dependent.	bind
6805	4	2913	6	10	NULL	NULL	NULL	statement 2	Process		is dependent on					time	Time				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1589_1_31_s_140	11909639	(A) Inhibition of ALDO binding to MR by PLP is concentration- and time-dependent.	bind
6406	1	2914	5	10	NULL	NULL	NULL	BMP-7	GP		bind					ROS 17/2	Cell				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_308_4_858_s_192	12927798	(A) Inhibition of BMP-7 binding to ROS 17/2.	bind
6810	1	2914	6	10	NULL	NULL	NULL	BMP-7	GP		bind					ROS 17/2	Cell				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_308_4_858_s_192	12927798	(A) Inhibition of BMP-7 binding to ROS 17/2.	bind
7118	1	2915	5	10	NULL	NULL	NULL	TCP	Chemical		bind					NMDA receptors	GP		NR2B subunit		NULL	rat brain membranes	NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_296_1_150_s_123	11123375	(A) inhibition of NR1a/2B receptors expressed in  Xenopus oocytes or (B) inhibition of [3]TCP binding to NR2B subunit containing NMDA receptors in rat brain membranes or (C) inhibition of [3]DTG binding to sigma sites in rat brain membranes.	bind
7119	2	2915	5	10	NULL	NULL	NULL	DTG	Chemical		bind								sigma sites		NULL	rat brain membrane	NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_296_1_150_s_123	11123375	(A) inhibition of NR1a/2B receptors expressed in  Xenopus oocytes or (B) inhibition of [3]TCP binding to NR2B subunit containing NMDA receptors in rat brain membranes or (C) inhibition of [3]DTG binding to sigma sites in rat brain membranes.	bind
46558	3	2915	5	10	NULL	NULL	NULL	NR1a/2B receptors	GP		is expressed in					 oocytes	Cell	Xenopus			NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_296_1_150_s_123	11123375	(A) inhibition of NR1a/2B receptors expressed in  Xenopus oocytes or (B) inhibition of [3]TCP binding to NR2B subunit containing NMDA receptors in rat brain membranes or (C) inhibition of [3]DTG binding to sigma sites in rat brain membranes.	bind
6811	1	2915	6	10	NULL	NULL	NULL	NR1a/2B receptors	GP		expressed in					oocytes	Cell	Xenopus			NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_296_1_150_s_123	11123375	(A) inhibition of NR1a/2B receptors expressed in  Xenopus oocytes or (B) inhibition of [3]TCP binding to NR2B subunit containing NMDA receptors in rat brain membranes or (C) inhibition of [3]DTG binding to sigma sites in rat brain membranes.	bind
6813	3	2915	6	10	NULL	NULL	NULL	TCP	Chemical		bind					NMDA receptors	GP		NR2B subunit		NULL	rat brain membranes	NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_296_1_150_s_123	11123375	(A) inhibition of NR1a/2B receptors expressed in  Xenopus oocytes or (B) inhibition of [3]TCP binding to NR2B subunit containing NMDA receptors in rat brain membranes or (C) inhibition of [3]DTG binding to sigma sites in rat brain membranes.	bind
6814	2	2915	6	10	NULL	NULL	NULL	DTG	Chemical		bind								sigma sites 		NULL	rat brain membranes	NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_296_1_150_s_123	11123375	(A) inhibition of NR1a/2B receptors expressed in  Xenopus oocytes or (B) inhibition of [3]TCP binding to NR2B subunit containing NMDA receptors in rat brain membranes or (C) inhibition of [3]DTG binding to sigma sites in rat brain membranes.	bind
6413	1	2916	5	10	NULL	NULL	NULL	peptide V	AminoAcid		mediate					LDL	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_4_753_s_286	10191300	(A) Inhibition of peptide V-mediated binding of LDL by LDL, HDL, and AcLDL.	bind
6414	2	2916	5	10	NULL	NULL	NULL	LDL	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_4_753_s_286	10191300	(A) Inhibition of peptide V-mediated binding of LDL by LDL, HDL, and AcLDL.	bind
6415	3	2916	5	10	NULL	NULL	NULL	HDL	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_4_753_s_286	10191300	(A) Inhibition of peptide V-mediated binding of LDL by LDL, HDL, and AcLDL.	bind
6416	4	2916	5	10	NULL	NULL	NULL	AcLDL	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_4_753_s_286	10191300	(A) Inhibition of peptide V-mediated binding of LDL by LDL, HDL, and AcLDL.	bind
6817	1	2916	6	10	NULL	NULL	NULL	peptide V	AminoAcid		mediates					LDL	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_4_753_s_286	10191300	(A) Inhibition of peptide V-mediated binding of LDL by LDL, HDL, and AcLDL.	bind
6819	2	2916	6	10	NULL	NULL	NULL	LDL	Chemical		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_4_753_s_286	10191300	(A) Inhibition of peptide V-mediated binding of LDL by LDL, HDL, and AcLDL.	bind
6820	3	2916	6	10	NULL	NULL	NULL	HDL	Chemical		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_4_753_s_286	10191300	(A) Inhibition of peptide V-mediated binding of LDL by LDL, HDL, and AcLDL.	bind
6825	4	2916	6	10	NULL	NULL	NULL	AcLDL	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_4_753_s_286	10191300	(A) Inhibition of peptide V-mediated binding of LDL by LDL, HDL, and AcLDL.	bind
7120	1	2917	5	10	NULL	NULL	NULL	K2-3f	GP		bind			scFv		Ab1 mAb K2-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1638_3_257_s_276	12878327	(A) Inhibition of scFv K2-3f binding to Ab1 mAb K2-3 by cocaine.	bind
7121	2	2917	5	10	NULL	NULL	NULL	cocaine	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1638_3_257_s_276	12878327	(A) Inhibition of scFv K2-3f binding to Ab1 mAb K2-3 by cocaine.	bind
6918	1	2917	6	10	NULL	NULL	NULL	K2-3f	GP		bind			scFv		Ab1 mAb K2-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1638_3_257_s_276	12878327	(A) Inhibition of scFv K2-3f binding to Ab1 mAb K2-3 by cocaine.	bind
6919	2	2917	6	10	NULL	NULL	NULL	cocaine	Chemical		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1638_3_257_s_276	12878327	(A) Inhibition of scFv K2-3f binding to Ab1 mAb K2-3 by cocaine.	bind
6443	1	2918	5	10	NULL	NULL	NULL	mAb	GP		bind					TcP2	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_301_4_819_s_65	12589786	(A) Inhibition of the  binding of mAb to TcP2  by scFv. TcP2 -coated plates were incubated with different  concentrations of scFv alone, scFv plus R13, or scFv plus TMVP.	bind
6444	2	2918	5	10	NULL	NULL	NULL	scFv	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_301_4_819_s_65	12589786	(A) Inhibition of the  binding of mAb to TcP2  by scFv. TcP2 -coated plates were incubated with different  concentrations of scFv alone, scFv plus R13, or scFv plus TMVP.	bind
6920	1	2918	6	10	NULL	NULL	NULL	mAb	GP		bind					TcP2	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_301_4_819_s_65	12589786	(A) Inhibition of the  binding of mAb to TcP2  by scFv. TcP2 -coated plates were incubated with different  concentrations of scFv alone, scFv plus R13, or scFv plus TMVP.	bind
6921	2	2918	6	10	NULL	NULL	NULL	scFv	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_301_4_819_s_65	12589786	(A) Inhibition of the  binding of mAb to TcP2  by scFv. TcP2 -coated plates were incubated with different  concentrations of scFv alone, scFv plus R13, or scFv plus TMVP.	bind
6445	1	2919	5	10	NULL	NULL	NULL	mAb	GP		bind					TcP2	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_301_4_819_s_65	12589786	(A) Inhibition of the binding of mAb to TcP2  by scFv. TcP2 -coated plates were incubated with different concentrations of scFv alone, scFv plus R13, or scFv plus TMVP.	bind
6446	2	2919	5	10	NULL	NULL	NULL	scFv	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_301_4_819_s_65	12589786	(A) Inhibition of the binding of mAb to TcP2  by scFv. TcP2 -coated plates were incubated with different concentrations of scFv alone, scFv plus R13, or scFv plus TMVP.	bind
6922	1	2919	6	10	NULL	NULL	NULL	mAb	GP		bind					TcP2	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_301_4_819_s_65	12589786	(A) Inhibition of the binding of mAb to TcP2  by scFv. TcP2 -coated plates were incubated with different concentrations of scFv alone, scFv plus R13, or scFv plus TMVP.	bind
6923	2	2919	6	10	NULL	NULL	NULL	scFv	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_301_4_819_s_65	12589786	(A) Inhibition of the binding of mAb to TcP2  by scFv. TcP2 -coated plates were incubated with different concentrations of scFv alone, scFv plus R13, or scFv plus TMVP.	bind
6447	1	2920	5	10	NULL	NULL	NULL	SOCS-1	GP		bind					IR	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_12_5434_s_147	15169905	(a) Insulin-dependent binding of SOCS-1  and SOCS-3 to the IR in vivo.	bind
6448	2	2920	5	10	NULL	NULL	NULL	statement 1	Process		is dependent on					insulin	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_12_5434_s_147	15169905	(a) Insulin-dependent binding of SOCS-1  and SOCS-3 to the IR in vivo.	bind
6449	3	2920	5	10	NULL	NULL	NULL	SOCS-3	GP		bind					IR	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_12_5434_s_147	15169905	(a) Insulin-dependent binding of SOCS-1  and SOCS-3 to the IR in vivo.	bind
6450	4	2920	5	10	NULL	NULL	NULL	statement 3	Process		is dependent on					insulin	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_12_5434_s_147	15169905	(a) Insulin-dependent binding of SOCS-1  and SOCS-3 to the IR in vivo.	bind
6924	1	2920	6	10	NULL	NULL	NULL	SOCS-1	GP		bind					IR	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_12_5434_s_147	15169905	(a) Insulin-dependent binding of SOCS-1  and SOCS-3 to the IR in vivo.	bind
6925	2	2920	6	10	NULL	NULL	NULL	SOCS-3	GP		bind					IR	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_12_5434_s_147	15169905	(a) Insulin-dependent binding of SOCS-1  and SOCS-3 to the IR in vivo.	bind
6926	3	2920	6	10	NULL	NULL	NULL	statement 1	Process		is dependent on					insulin	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_12_5434_s_147	15169905	(a) Insulin-dependent binding of SOCS-1  and SOCS-3 to the IR in vivo.	bind
6927	4	2920	6	10	NULL	NULL	NULL	statement 2	Process		is dependent on					insulin	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_12_5434_s_147	15169905	(a) Insulin-dependent binding of SOCS-1  and SOCS-3 to the IR in vivo.	bind
6451	1	2921	5	10	NULL	NULL	NULL	Val-tRNAIle	NucleicAcid		interact with					IleRS	GP		editing domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_103_5_793_s_170	11114335	(A) Interactions  of the Val-tRNAIle with the IleRS editing domain at the posttransfer editing  step.	bind
6452	2	2921	5	10	NULL	NULL	NULL	statement 1	Process		occurs at					posttransfer editing step	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_5_793_s_170	11114335	(A) Interactions  of the Val-tRNAIle with the IleRS editing domain at the posttransfer editing  step.	bind
6928	1	2921	6	10	NULL	NULL	NULL	Val-tRNAIle	NucleicAcid		interact with					IleRS	GP		editing domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_103_5_793_s_170	11114335	(A) Interactions  of the Val-tRNAIle with the IleRS editing domain at the posttransfer editing  step.	bind
6929	2	2921	6	10	NULL	NULL	NULL	statement 1	Process		occurs at					posttransfer editing step	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_5_793_s_170	11114335	(A) Interactions  of the Val-tRNAIle with the IleRS editing domain at the posttransfer editing  step.	bind
6453	1	2922	5	10	NULL	NULL	NULL	BTX BR36	GP		interacts with					AChR	GP		ACh binding pocket		NULL		NULL	NULL	NULL	NULL	gw60_neuron_35_2_319_s_171	12160749	(A) Interactions of  -BTX BR36 (blue) in the ACh binding pocket of AChR at the interface between the  1 and   subunits and (B) at the interface between the  1 and   subunits.	bind
7123	2	2922	5	10	NULL	NULL	NULL	statement 1	Process		occurs at								interface between 1 and subunits		NULL		NULL	NULL	NULL	NULL	gw60_neuron_35_2_319_s_171	12160749	(A) Interactions of  -BTX BR36 (blue) in the ACh binding pocket of AChR at the interface between the  1 and   subunits and (B) at the interface between the  1 and   subunits.	bind
7020	1	2922	6	10	NULL	NULL	NULL	BTX Br36	GP		interacts with					AChR	GP		ACh binding pocket		NULL		NULL	NULL	NULL	NULL	gw60_neuron_35_2_319_s_171	12160749	(A) Interactions of  -BTX BR36 (blue) in the ACh binding pocket of AChR at the interface between the  1 and   subunits and (B) at the interface between the  1 and   subunits.	bind
7021	2	2922	6	10	NULL	NULL	NULL	statement 1	Process		occurs at								interface between the 1 and subunits		NULL		NULL	NULL	NULL	NULL	gw60_neuron_35_2_319_s_171	12160749	(A) Interactions of  -BTX BR36 (blue) in the ACh binding pocket of AChR at the interface between the  1 and   subunits and (B) at the interface between the  1 and   subunits.	bind
6454	1	2923	5	10	NULL	NULL	NULL	Iqg1p	GP		bind					Sec3p	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_4_601_s_130	12446742	(A) Iqg1p binds Sec3p.	bind
6935	1	2923	6	10	NULL	NULL	NULL	Iqg1p	GP		bind					Sec3p	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_4_601_s_130	12446742	(A) Iqg1p binds Sec3p.	bind
6455	1	2924	5	10	NULL	NULL	NULL	SR	GP		bind			 SRX domain		GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_6_793_s_208	12654246	(A) Isothermal calorimetric titration of SR  bound to GTP (cyan diamonds) or GDP (magenta diamonds) with the SRX domain of SR .	bind
6456	2	2924	5	10	NULL	NULL	NULL	SR	GP		bind			 SRX domain		GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_6_793_s_208	12654246	(A) Isothermal calorimetric titration of SR  bound to GTP (cyan diamonds) or GDP (magenta diamonds) with the SRX domain of SR .	bind
46559	3	2924	5	10	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_6_793_s_208	12654246	(A) Isothermal calorimetric titration of SR  bound to GTP (cyan diamonds) or GDP (magenta diamonds) with the SRX domain of SR .	bind
6939	1	2924	6	10	NULL	NULL	NULL	SR	GP		bind			SRX domain		GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_6_793_s_208	12654246	(A) Isothermal calorimetric titration of SR  bound to GTP (cyan diamonds) or GDP (magenta diamonds) with the SRX domain of SR .	bind
6940	2	2924	6	10	NULL	NULL	NULL	SR	GP		bind			SRX domain		GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_6_793_s_208	12654246	(A) Isothermal calorimetric titration of SR  bound to GTP (cyan diamonds) or GDP (magenta diamonds) with the SRX domain of SR .	bind
46560	3	2924	6	10	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_6_793_s_208	12654246	(A) Isothermal calorimetric titration of SR  bound to GTP (cyan diamonds) or GDP (magenta diamonds) with the SRX domain of SR .	bind
6457	1	2925	5	10	NULL	NULL	NULL	Abl	GP	purified	bind			kinase domain		c-Abl 1b peptide	AminoAcid	myristoylated	Myr-GQQPGKVLGDQRRPSL		NULL		NULL	NULL	NULL	NULL	gw60_cell_112_6_845_s_67	12654250	(A) Isothermal titration calorimetry measuring binding of the purified Abl kinase domain to a myristoylated c-Abl 1b peptide (Myr-GQQPGKVLGDQRRPSL).	bind
6945	1	2925	6	10	NULL	NULL	NULL	Abl 	GP	purified	bind			kinase domain		c-Abl 1b peptide	AminoAcid	myristoylated	Myr-GQQPGKVLGDQRRPSL		NULL		NULL	NULL	NULL	NULL	gw60_cell_112_6_845_s_67	12654250	(A) Isothermal titration calorimetry measuring binding of the purified Abl kinase domain to a myristoylated c-Abl 1b peptide (Myr-GQQPGKVLGDQRRPSL).	bind
6474	1	2926	5	10	NULL	NULL	NULL	paxillin	GP		bind					alpha4	GP		tail		NULL	JB4 cells	NULL	NULL	NULL	NULL	gw70_cellbiol_171_6_1073_s_75	16365170	(A) JB4 cells expressing either wt alpha4 or alpha4(Y991A) were pretreated for 15 min with A7B7C7, a cell-permeable inhibitor of paxillin  binding to the alpha4 tail, or with the control compound A6B6C6, both present at 5 muM.	bind
6475	2	2926	5	10	NULL	NULL	NULL	A7B7C7	Chemical		inhibit					statement 1	Process				NULL	JB4 cells	NULL	NULL	NULL	NULL	gw70_cellbiol_171_6_1073_s_75	16365170	(A) JB4 cells expressing either wt alpha4 or alpha4(Y991A) were pretreated for 15 min with A7B7C7, a cell-permeable inhibitor of paxillin  binding to the alpha4 tail, or with the control compound A6B6C6, both present at 5 muM.	bind
46799	3	2926	5	10	NULL	NULL	NULL	A7B7C7	Chemical		is a type of					cell-permeable inhibitor	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_6_1073_s_75	16365170	(A) JB4 cells expressing either wt alpha4 or alpha4(Y991A) were pretreated for 15 min with A7B7C7, a cell-permeable inhibitor of paxillin  binding to the alpha4 tail, or with the control compound A6B6C6, both present at 5 muM.	bind
7024	1	2926	6	10	NULL	NULL	NULL	paxillin	GP		bind					alpha-4	GP		tail		NULL	JB4 cells	NULL	NULL	NULL	NULL	gw70_cellbiol_171_6_1073_s_75	16365170	(A) JB4 cells expressing either wt alpha4 or alpha4(Y991A) were pretreated for 15 min with A7B7C7, a cell-permeable inhibitor of paxillin  binding to the alpha4 tail, or with the control compound A6B6C6, both present at 5 muM.	bind
7025	2	2926	6	10	NULL	NULL	NULL	A7B7C7	Chemical		inhibits					statement 1	Process				NULL	JB4 cells	NULL	NULL	NULL	NULL	gw70_cellbiol_171_6_1073_s_75	16365170	(A) JB4 cells expressing either wt alpha4 or alpha4(Y991A) were pretreated for 15 min with A7B7C7, a cell-permeable inhibitor of paxillin  binding to the alpha4 tail, or with the control compound A6B6C6, both present at 5 muM.	bind
46800	3	2926	6	10	NULL	NULL	NULL	A7B7C7	Chemical		is a type of 					cell-permeable inhibitor	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_6_1073_s_75	16365170	(A) JB4 cells expressing either wt alpha4 or alpha4(Y991A) were pretreated for 15 min with A7B7C7, a cell-permeable inhibitor of paxillin  binding to the alpha4 tail, or with the control compound A6B6C6, both present at 5 muM.	bind
6476	1	2927	5	10	NULL	NULL	NULL	JDP2	GP		bind					ATF-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4815_s_86	12052888	(A) JDP2 binds to DRE as a heterodimer with ATF-2.	bind
6477	2	2927	5	10	NULL	NULL	NULL	statement 1	Process		bind									DRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4815_s_86	12052888	(A) JDP2 binds to DRE as a heterodimer with ATF-2.	bind
6950	1	2927	6	10	NULL	NULL	NULL	JDP2	GP		bind					ATF-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4815_s_86	12052888	(A) JDP2 binds to DRE as a heterodimer with ATF-2.	bind
6951	2	2927	6	10	NULL	NULL	NULL	statement 1	Process		forms a 					heterodimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4815_s_86	12052888	(A) JDP2 binds to DRE as a heterodimer with ATF-2.	bind
6954	3	2927	6	10	NULL	NULL	NULL	statement 2	Process		bind									DRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4815_s_86	12052888	(A) JDP2 binds to DRE as a heterodimer with ATF-2.	bind
6478	1	2929	5	10	NULL	NULL	NULL	Kalirin	GP		bind					PAM-CD/GST	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_3_629_s_129	11251076	(A) Kalirin binding to mutant PAM-CD/GST fusion proteins: CHO cells stably expressing  myc.	bind
46561	2	2929	5	10	NULL	NULL	NULL	CHO cells	Cell		express		stably			myc	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_3_629_s_129	11251076	(A) Kalirin binding to mutant PAM-CD/GST fusion proteins: CHO cells stably expressing  myc.	bind
67056	3	2929	5	10	NULL	0	NULL	PAM-CD/GST	GP		is a type of					fusion protein	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_3_629_s_129	11251076	(A) Kalirin binding to mutant PAM-CD/GST fusion proteins: CHO cells stably expressing  myc.	bind
6959	1	2929	6	10	NULL	NULL	NULL	Kalirin	GP		bind					PAM-CD/GST	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_3_629_s_129	11251076	(A) Kalirin binding to mutant PAM-CD/GST fusion proteins: CHO cells stably expressing  myc.	bind
6960	2	2929	6	10	NULL	NULL	NULL	CHO cells	Cell		express		stably			myc	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_3_629_s_129	11251076	(A) Kalirin binding to mutant PAM-CD/GST fusion proteins: CHO cells stably expressing  myc.	bind
67057	3	2929	6	10	NULL	0	NULL	PAM-CD/GST	GP		is a type of					fusion protein	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_3_629_s_129	11251076	(A) Kalirin binding to mutant PAM-CD/GST fusion proteins: CHO cells stably expressing  myc.	bind
6479	1	2930	5	10	NULL	NULL	NULL	KdgR	GP		bind					eda	GP			P2 promoter 	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_187_3_991_s_202	15659677	(A) KdgR binding to the  eda P2 promoter region.	bind
6961	1	2930	6	10	NULL	NULL	NULL	KdgR	GP		bind					eda	GP			P2 promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_187_3_991_s_202	15659677	(A) KdgR binding to the  eda P2 promoter region.	bind
6480	1	2931	5	10	NULL	NULL	NULL	P6EtG/HLA-A2	GP		bind					A6	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_13_4_475_s_106	11070166	(A) Kinetic data for P6EtG/HLA-A2 binding to A6.	bind
6964	1	2931	6	10	NULL	NULL	NULL	P6EtG/HLA-A2	GP		bind					A6	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_13_4_475_s_106	11070166	(A) Kinetic data for P6EtG/HLA-A2 binding to A6.	bind
6483	1	2933	5	10	NULL	NULL	NULL	12aa(+PO4) peptide	AminoAcid		bind					Nck	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_3_407_s_172	14757753	(A) Latex beads were coated with 12aa(+PO4), a peptide that binds human Nck; 12aa, a nonphosphorylated peptide that lacks Nck-binding  activity; or 7aa(+PO4), a peptide that binds Nck poorly ( ).	bind
6484	2	2933	5	10	NULL	NULL	NULL	12aa peptide	AminoAcid	nonphosphorylated	lacks					Nck	GP	human;;binding activity of			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_3_407_s_172	14757753	(A) Latex beads were coated with 12aa(+PO4), a peptide that binds human Nck; 12aa, a nonphosphorylated peptide that lacks Nck-binding  activity; or 7aa(+PO4), a peptide that binds Nck poorly ( ).	bind
6485	3	2933	5	10	NULL	NULL	NULL	7aa(+PO4) peptide	AminoAcid		bind		poorly			Nck	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_3_407_s_172	14757753	(A) Latex beads were coated with 12aa(+PO4), a peptide that binds human Nck; 12aa, a nonphosphorylated peptide that lacks Nck-binding  activity; or 7aa(+PO4), a peptide that binds Nck poorly ( ).	bind
6965	1	2933	6	10	NULL	NULL	NULL	 12aa(+PO4) peptide	AminoAcid		bind					Nck	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_3_407_s_172	14757753	(A) Latex beads were coated with 12aa(+PO4), a peptide that binds human Nck; 12aa, a nonphosphorylated peptide that lacks Nck-binding  activity; or 7aa(+PO4), a peptide that binds Nck poorly ( ).	bind
6966	2	2933	6	10	NULL	NULL	NULL	12aa peptide	AminoAcid	nonphosphorylated	lacks					Nck	GP	human;;binding activity of			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_3_407_s_172	14757753	(A) Latex beads were coated with 12aa(+PO4), a peptide that binds human Nck; 12aa, a nonphosphorylated peptide that lacks Nck-binding  activity; or 7aa(+PO4), a peptide that binds Nck poorly ( ).	bind
6967	3	2933	6	10	NULL	NULL	NULL	7aa(+PO4) peptide	AminoAcid		bind		poorly			Nck	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_3_407_s_172	14757753	(A) Latex beads were coated with 12aa(+PO4), a peptide that binds human Nck; 12aa, a nonphosphorylated peptide that lacks Nck-binding  activity; or 7aa(+PO4), a peptide that binds Nck poorly ( ).	bind
6481	1	2937	5	10	NULL	NULL	NULL	Ras	GP		bind					Raf-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_24_8_1353_s_88	12807734	(A) Levels of Ras bound  to Raf-1.	bind
6968	1	2937	6	10	NULL	NULL	NULL	Ras	GP		bind					Raf-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_24_8_1353_s_88	12807734	(A) Levels of Ras bound  to Raf-1.	bind
6482	1	2938	5	10	NULL	NULL	NULL	Ras	GP		bind					Raf-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_carcinogenesis_24_8_1353_s_88	12807734	(A) Levels of Ras bound to Raf-1.	bind
6969	1	2938	6	10	NULL	NULL	NULL	Ras	GP		bind					Raf-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_carcinogenesis_24_8_1353_s_88	12807734	(A) Levels of Ras bound to Raf-1.	bind
6486	1	2940	5	10	NULL	NULL	NULL	LIN-1	GP		bind					LIN-31	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_cell_93_4_569_s_101	9604932	(A) LIN-1 binds  to LIN-31 in vivo.	bind
6970	1	2940	6	10	NULL	NULL	NULL	LIN-1	GP		bind					LIN-31	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_cell_93_4_569_s_101	9604932	(A) LIN-1 binds  to LIN-31 in vivo.	bind
6488	1	2941	5	10	NULL	NULL	NULL	pAFS60 plasmid	NucleicAcid	2mum-based	carry									lac operator repeats	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4218_s_186	12024034	(A) Localization of 2mum-based plasmid pAFS60, which carries  lac operator repeats that bind GFP-Lacr fusion protein.	bind
6489	2	2941	5	10	NULL	NULL	NULL	statement 1	Process		bind					GFP-Lacr	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4218_s_186	12024034	(A) Localization of 2mum-based plasmid pAFS60, which carries  lac operator repeats that bind GFP-Lacr fusion protein.	bind
67058	3	2941	5	10	NULL	0	NULL	GFP-Lacr	GP		is a type of					fusion protein	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_12_4218_s_186	12024034	(A) Localization of 2mum-based plasmid pAFS60, which carries  lac operator repeats that bind GFP-Lacr fusion protein.	bind
6971	1	2941	6	10	NULL	NULL	NULL	plasmid pAFS60	NucleicAcid		carry									lac operator repeats	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4218_s_186	12024034	(A) Localization of 2mum-based plasmid pAFS60, which carries  lac operator repeats that bind GFP-Lacr fusion protein.	bind
6972	2	2941	6	10	NULL	NULL	NULL	statement 1	Process		bind					GFP-Lacr	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4218_s_186	12024034	(A) Localization of 2mum-based plasmid pAFS60, which carries  lac operator repeats that bind GFP-Lacr fusion protein.	bind
67059	3	2941	6	10	NULL	0	NULL	GFP-Lacr	GP		is a type of					fusion protein	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_12_4218_s_186	12024034	(A) Localization of 2mum-based plasmid pAFS60, which carries  lac operator repeats that bind GFP-Lacr fusion protein.	bind
6492	1	2942	5	10	NULL	NULL	NULL	Pan3p	GP		bind					Pab1p	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_12_5521_s_216	15169912	(A) Location in the primary  structure of Pab1p of point mutants that alter Pan3p binding to Pab1p.	bind
6493	2	2942	5	10	NULL	NULL	NULL	Pab1p	GP	point mutants	alter					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_12_5521_s_216	15169912	(A) Location in the primary  structure of Pab1p of point mutants that alter Pan3p binding to Pab1p.	bind
6973	1	2942	6	10	NULL	NULL	NULL	Pan3p	GP		bind					Pab1p	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_12_5521_s_216	15169912	(A) Location in the primary  structure of Pab1p of point mutants that alter Pan3p binding to Pab1p.	bind
6974	2	2942	6	10	NULL	NULL	NULL	Pab1p	GP	point mutant	alters					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_12_5521_s_216	15169912	(A) Location in the primary  structure of Pab1p of point mutants that alter Pan3p binding to Pab1p.	bind
7128	1	2944	5	10	NULL	NULL	NULL	IRES	GP	wild type	bind			loop between J and K domains		eIF4G	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_29_18599_s_99	9660832	(A) loop between J and K domains that is bound by eIF4G in the wild type IRES is intact in this mutant (Fig.  3 A).	bind
6975	1	2944	6	10	NULL	NULL	NULL	eIF4G	GP		bind					IRES	GP	wild type	loop betweeJ and K domains		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_29_18599_s_99	9660832	(A) loop between J and K domains that is bound by eIF4G in the wild type IRES is intact in this mutant (Fig.  3 A).	bind
7129	1	2945	5	10	NULL	NULL	NULL	basal transcription	Process	low level of	in the absence of					AfaF	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_6_1886_s_227	12618452	(A) Low level of basal transcription in the absence of AfaF and alanine; GATCdist is methylated, whereas Lrp is bound to GATCprox; ClpB is bound near to the promoter region.	bind
7130	2	2945	5	10	NULL	NULL	NULL	basal transcription	Process	low level of	in the absence of								alanine		NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_6_1886_s_227	12618452	(A) Low level of basal transcription in the absence of AfaF and alanine; GATCdist is methylated, whereas Lrp is bound to GATCprox; ClpB is bound near to the promoter region.	bind
7131	3	2945	5	10	NULL	NULL	NULL				undergoes				GATCdist	methylation	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_6_1886_s_227	12618452	(A) Low level of basal transcription in the absence of AfaF and alanine; GATCdist is methylated, whereas Lrp is bound to GATCprox; ClpB is bound near to the promoter region.	bind
7132	4	2945	5	10	NULL	NULL	NULL	Lrp	GP		bind									GATCprox	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_6_1886_s_227	12618452	(A) Low level of basal transcription in the absence of AfaF and alanine; GATCdist is methylated, whereas Lrp is bound to GATCprox; ClpB is bound near to the promoter region.	bind
7133	5	2945	5	10	NULL	NULL	NULL	ClpB	GP		bind									near to promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_6_1886_s_227	12618452	(A) Low level of basal transcription in the absence of AfaF and alanine; GATCdist is methylated, whereas Lrp is bound to GATCprox; ClpB is bound near to the promoter region.	bind
6976	1	2945	6	10	NULL	NULL	NULL	Lrp	GP		bind									GATCprox	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_6_1886_s_227	12618452	(A) Low level of basal transcription in the absence of AfaF and alanine; GATCdist is methylated, whereas Lrp is bound to GATCprox; ClpB is bound near to the promoter region.	bind
6977	2	2945	6	10	NULL	NULL	NULL				undergoes				GATCdist	methylation	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_6_1886_s_227	12618452	(A) Low level of basal transcription in the absence of AfaF and alanine; GATCdist is methylated, whereas Lrp is bound to GATCprox; ClpB is bound near to the promoter region.	bind
6978	3	2945	6	10	NULL	NULL	NULL	ClpB	GP		bind									near to the promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_6_1886_s_227	12618452	(A) Low level of basal transcription in the absence of AfaF and alanine; GATCdist is methylated, whereas Lrp is bound to GATCprox; ClpB is bound near to the promoter region.	bind
46562	4	2945	6	10	NULL	NULL	NULL	basal transcription	Process	low level of 	in the absence of					AfaF	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_6_1886_s_227	12618452	(A) Low level of basal transcription in the absence of AfaF and alanine; GATCdist is methylated, whereas Lrp is bound to GATCprox; ClpB is bound near to the promoter region.	bind
46563	5	2945	6	10	NULL	NULL	NULL	basal transcription	Process	low level of	in the absence of								alanine		NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_6_1886_s_227	12618452	(A) Low level of basal transcription in the absence of AfaF and alanine; GATCdist is methylated, whereas Lrp is bound to GATCprox; ClpB is bound near to the promoter region.	bind
6494	1	2946	5	10	NULL	NULL	NULL	Fli-I	GP		bind			LRR domain		GRIP1	GP		N-terminal region		NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_5_2103_s_268	14966289	(A) LRR domain of Fli-I binds to GRIP1 N-terminal region in vitro.	bind
6979	1	2946	6	10	NULL	NULL	NULL	Fli-I	GP		bind			LRR domain		GRIP1	GP		N-terminal region		NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_5_2103_s_268	14966289	(A) LRR domain of Fli-I binds to GRIP1 N-terminal region in vitro.	bind
6495	1	2947	5	10	NULL	0	NULL		NULL		bind	NULL		Ly49C		Kb molecules	NULL				NULL	lymphoblasts	NULL	NULL	NULL	NULL	gw60_immunity_11_1_67_s_110	10435580	(A) Ly49C and Ly49I bind to Kb molecules on lymphoblasts but not appreciably to Db molecules.	bind
6499	2	2947	5	NULL	NULL	0	NULL		NULL		bind	NULL	not appreciable	Ly49C		Db molecules	NULL				NULL		0	NULL	NULL	NULL	gw60_immunity_11_1_67_s_110	10435580	(A) Ly49C and Ly49I bind to Kb molecules on lymphoblasts but not appreciably to Db molecules.	bind
6501	3	2947	5	10	NULL	0	NULL		NULL		bind	NULL		Ly49I		Kb molecules	NULL				NULL	lymphoblasts	NULL	NULL	NULL	NULL	gw60_immunity_11_1_67_s_110	10435580	(A) Ly49C and Ly49I bind to Kb molecules on lymphoblasts but not appreciably to Db molecules.	bind
6502	4	2947	5	NULL	NULL	0	NULL		NULL		bind	NULL	not appreciable	Ly49I		Db molecules	NULL				NULL		0	NULL	NULL	NULL	gw60_immunity_11_1_67_s_110	10435580	(A) Ly49C and Ly49I bind to Kb molecules on lymphoblasts but not appreciably to Db molecules.	bind
6980	1	2947	6	NULL	NULL	0	NULL		NULL		bind	NULL		Ly49C		Kb molecules	NULL				NULL	lymphoblasts	0	NULL	NULL	NULL	gw60_immunity_11_1_67_s_110	10435580	(A) Ly49C and Ly49I bind to Kb molecules on lymphoblasts but not appreciably to Db molecules.	bind
6981	2	2947	6	NULL	NULL	0	NULL		NULL		bind	NULL		Ly49I		Kb molecules	NULL				NULL	lymphoblasts	0	NULL	NULL	NULL	gw60_immunity_11_1_67_s_110	10435580	(A) Ly49C and Ly49I bind to Kb molecules on lymphoblasts but not appreciably to Db molecules.	bind
6982	3	2947	6	NULL	NULL	0	NULL		NULL		bind	NULL	not appreciably	Ly49C		Db molecules	NULL				NULL	lymphoblasts	NULL	NULL	NULL	NULL	gw60_immunity_11_1_67_s_110	10435580	(A) Ly49C and Ly49I bind to Kb molecules on lymphoblasts but not appreciably to Db molecules.	bind
6983	4	2947	6	NULL	NULL	0	NULL		NULL		bind	NULL	not appreciably	Ly49I		Db molecules	NULL				NULL	lymphoblasts	NULL	NULL	NULL	NULL	gw60_immunity_11_1_67_s_110	10435580	(A) Ly49C and Ly49I bind to Kb molecules on lymphoblasts but not appreciably to Db molecules.	bind
6506	1	2949	5	10	NULL	NULL	NULL	Mad2	GP		bind					Mad1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_2_153_s_71	16636141	(A) Mad2 binds to Mad1 and adopts the N2'' conformation.	bind
6508	2	2949	5	10	NULL	NULL	NULL	statement 1	Process		adopt					N2'' conformation					NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_2_153_s_71	16636141	(A) Mad2 binds to Mad1 and adopts the N2'' conformation.	bind
53113	3	2949	5	10	NULL	NULL	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_2_153_s_71	16636141	(A) Mad2 binds to Mad1 and adopts the N2'' conformation.	bind
6984	1	2949	6	10	NULL	NULL	NULL	Mad2	GP		bind					Mad1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_2_153_s_71	16636141	(A) Mad2 binds to Mad1 and adopts the N2'' conformation.	bind
6985	2	2949	6	10	NULL	NULL	NULL	Mad2	GP		adopts					N2'' conformation					NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_2_153_s_71	16636141	(A) Mad2 binds to Mad1 and adopts the N2'' conformation.	bind
6986	3	2949	6	10	NULL	NULL	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_2_153_s_71	16636141	(A) Mad2 binds to Mad1 and adopts the N2'' conformation.	bind
6570	1	2950	5	10	NULL	NULL	NULL	MBP	GP		bind					maltose	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_5_1225_s_19	11844750	(A) MBP binds maltose, undergoing a change from an open conformation to a closed conformation, generating a high-affinity sugar-binding site.	bind
6571	2	2950	5	10	NULL	NULL	NULL	statement 1	Process	open conformation of	changes to					statement 1	Process	closed conformation of			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_5_1225_s_19	11844750	(A) MBP binds maltose, undergoing a change from an open conformation to a closed conformation, generating a high-affinity sugar-binding site.	bind
6572	3	2950	5	10	NULL	NULL	NULL	statement 2	Process		generate							high-affinity	sugar-binding site		NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_5_1225_s_19	11844750	(A) MBP binds maltose, undergoing a change from an open conformation to a closed conformation, generating a high-affinity sugar-binding site.	bind
6987	1	2950	6	10	NULL	NULL	NULL	MBP	GP		bind					maltose	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_5_1225_s_19	11844750	(A) MBP binds maltose, undergoing a change from an open conformation to a closed conformation, generating a high-affinity sugar-binding site.	bind
7026	2	2950	6	10	NULL	NULL	NULL	statement 1	Process	open conformation of	changes to					statement 1	Process	closed conformation of 			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_5_1225_s_19	11844750	(A) MBP binds maltose, undergoing a change from an open conformation to a closed conformation, generating a high-affinity sugar-binding site.	bind
7027	3	2950	6	10	NULL	NULL	NULL	statement 2	Process		generates							high-affinity	sugar binding site		NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_5_1225_s_19	11844750	(A) MBP binds maltose, undergoing a change from an open conformation to a closed conformation, generating a high-affinity sugar-binding site.	bind
6575	1	2955	5	10	NULL	NULL	NULL	MEF2	GP		bind		specifically			HRC	GP			MEF2 site	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_9_3757_s_210	15082771	(A) MEF2 binds specifically  to the HRC MEF2 site in vitro.	bind
6988	1	2955	6	10	NULL	NULL	NULL	MEF2	GP		bind		specifically			HRC	GP			MEF2 site 	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_9_3757_s_210	15082771	(A) MEF2 binds specifically  to the HRC MEF2 site in vitro.	bind
6576	1	2956	5	10	NULL	NULL	NULL	p24-32 peptide	AminoAcid		bind					H2-Dd	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_7_3829_s_152	15213124	(A) MHC class I stabilization assay indicated that the p24-32 peptide binds to H2-Dd.	bind
6989	1	2956	6	10	NULL	NULL	NULL	p24-32 peptide	AminoAcid		bind					H2-Dd	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_7_3829_s_152	15213124	(A) MHC class I stabilization assay indicated that the p24-32 peptide binds to H2-Dd.	bind
6578	1	2957	5	10	NULL	NULL	NULL	Mig6	GP		bind					Grb2	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_2_337_s_226	16247031	(A) Mig6 binds Grb2.	bind
6990	1	2957	6	10	NULL	NULL	NULL	Mig6	GP		bind					Grb2	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_2_337_s_226	16247031	(A) Mig6 binds Grb2.	bind
6579	1	2958	5	10	NULL	NULL	NULL	GRB2	GP	cotransfected	bind					p27	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_11_3735_s_179	12748278	(A) Mitogen stimulation enhances binding of cotransfected GRB2  and p27.	bind
6582	2	2958	5	10	NULL	NULL	NULL	mitogen	Chemical	stimulation	enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_11_3735_s_179	12748278	(A) Mitogen stimulation enhances binding of cotransfected GRB2  and p27.	bind
6991	1	2958	6	10	NULL	NULL	NULL	Grb2	GP		bind					p27	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_11_3735_s_179	12748278	(A) Mitogen stimulation enhances binding of cotransfected GRB2  and p27.	bind
6992	2	2958	6	10	NULL	NULL	NULL	mitogen	Chemical	stimulation of	enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_11_3735_s_179	12748278	(A) Mitogen stimulation enhances binding of cotransfected GRB2  and p27.	bind
6586	1	2960	5	10	NULL	NULL	NULL	Mlc1p	GP		bind					Myo1p	GP		IQ1		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_165_6_843_s_126	15210731	(A) Mlc1p binds to Myo1p through IQ1.	bind
6993	1	2960	6	10	NULL	NULL	NULL	Mlc1p	GP		bind					Myo1p	GP		IQ1		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_165_6_843_s_126	15210731	(A) Mlc1p binds to Myo1p through IQ1.	bind
6589	1	2961	5	10	NULL	NULL	NULL	MoB34	GP	purified from mouse ascites fluid	bind		dose dependently			NMGB bacteria	Organism				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_10_6399_s_209	16177311	(A) MoB34 purified from mouse ascites fluid bound to NMGB bacteria in dose-dependent  manner.	bind
6994	1	2961	6	10	NULL	NULL	NULL	MoB34	GP	purified from mouse ascites	bind		dose dependently			NMGB bacteria	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_10_6399_s_209	16177311	(A) MoB34 purified from mouse ascites fluid bound to NMGB bacteria in dose-dependent  manner.	bind
6592	1	2962	5	10	NULL	NULL	NULL	CRP	GP	E. coli	bind			recognition helix		DNA	NucleicAcid			half-side consensus sequence	NULL		NULL	NULL	NULL	NULL	gw70_febslett_571_1_154_s_175	15280034	(A) Mode  of binding between the recognition helix of  E. coli CRP and the half-side consensus DNA sequence.	bind
6996	1	2962	6	10	NULL	NULL	NULL	CRP	GP	E.coli	bind			recognition helix		DNA	NucleicAcid			half side consensus	NULL		NULL	NULL	NULL	NULL	gw70_febslett_571_1_154_s_175	15280034	(A) Mode  of binding between the recognition helix of  E. coli CRP and the half-side consensus DNA sequence.	bind
6597	1	2963	5	10	NULL	NULL	NULL	phosphoserine-proline dipeptide	AminoAcid		bind					Pin1	GP		active site		NULL		NULL	NULL	NULL	NULL	gw60_cell_89_6_875_s_168	9200606	(A) Model for a phosphoserine-proline dipeptide bound to Pin1's active site.	bind
6997	1	2963	6	10	NULL	NULL	NULL	phosphoserine-proline dipeptide	AminoAcid		bind					Pin1	GP		active site		NULL		NULL	NULL	NULL	NULL	gw60_cell_89_6_875_s_168	9200606	(A) Model for a phosphoserine-proline dipeptide bound to Pin1's active site.	bind
6599	1	2965	5	10	NULL	NULL	NULL	 9G11	GP		bind					CD31	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_5_316_s_124	9115397	(a) Monoclonal antibody 9G11 binding to CD31;  (b) rabbit polyclonal antibodies binding to P-selectin;  (c) monoclonal antibody 15.2 binding to ICAM-1.	bind
6601	2	2965	5	10	NULL	NULL	NULL	polyclonal antibodies	GP	rabbit	bind					P-selectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_5_316_s_124	9115397	(a) Monoclonal antibody 9G11 binding to CD31;  (b) rabbit polyclonal antibodies binding to P-selectin;  (c) monoclonal antibody 15.2 binding to ICAM-1.	bind
6602	3	2965	5	10	NULL	NULL	NULL	monoclonal antibody 15.2	GP		bind					ICAM-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_5_316_s_124	9115397	(a) Monoclonal antibody 9G11 binding to CD31;  (b) rabbit polyclonal antibodies binding to P-selectin;  (c) monoclonal antibody 15.2 binding to ICAM-1.	bind
53114	4	2965	5	10	NULL	NULL	NULL	9G11	GP		is a type of					monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_5_316_s_124	9115397	(a) Monoclonal antibody 9G11 binding to CD31;  (b) rabbit polyclonal antibodies binding to P-selectin;  (c) monoclonal antibody 15.2 binding to ICAM-1.	bind
6998	1	2965	6	10	NULL	NULL	NULL	 9G11	GP		bind					CD31	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_5_316_s_124	9115397	(a) Monoclonal antibody 9G11 binding to CD31;  (b) rabbit polyclonal antibodies binding to P-selectin;  (c) monoclonal antibody 15.2 binding to ICAM-1.	bind
6999	2	2965	6	10	NULL	NULL	NULL	polyclonal antibodies	GP	rabbit	bind					P-selectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_5_316_s_124	9115397	(a) Monoclonal antibody 9G11 binding to CD31;  (b) rabbit polyclonal antibodies binding to P-selectin;  (c) monoclonal antibody 15.2 binding to ICAM-1.	bind
7000	3	2965	6	10	NULL	NULL	NULL	monoclonal antibody 15.2	GP		bind					ICAM-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_5_316_s_124	9115397	(a) Monoclonal antibody 9G11 binding to CD31;  (b) rabbit polyclonal antibodies binding to P-selectin;  (c) monoclonal antibody 15.2 binding to ICAM-1.	bind
53115	4	2965	6	10	NULL	NULL	NULL	9G11	GP		is a type of					monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_5_316_s_124	9115397	(a) Monoclonal antibody 9G11 binding to CD31;  (b) rabbit polyclonal antibodies binding to P-selectin;  (c) monoclonal antibody 15.2 binding to ICAM-1.	bind
6606	1	2966	5	10	NULL	NULL	NULL	chromomycin A3	Chemical		bind		preferentially					viral		CRE flanking sequences	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_721_s_224	9447968	(A) MPE:Fe footprinting shows that chromomycin A3 binds preferentially to the viral CRE flanking sequences.	bind
7001	1	2966	6	10	NULL	NULL	NULL	chromomycin A3	Chemical		bind		preferentially					viral		CRE flanking sequences	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_721_s_224	9447968	(A) MPE:Fe footprinting shows that chromomycin A3 binds preferentially to the viral CRE flanking sequences.	bind
6607	1	2967	5	10	NULL	NULL	NULL	Munc13-1	GP		bind					RIM1	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_30_1_183_s_140	11343654	(A) Munc13-1 and Rab3A binding to RIM1 is mutually exclusive.	bind
6608	2	2967	5	10	NULL	NULL	NULL	Rab3A	GP		bind					RIM1	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_30_1_183_s_140	11343654	(A) Munc13-1 and Rab3A binding to RIM1 is mutually exclusive.	bind
6609	3	2967	5	10	NULL	NULL	NULL	statement 1	Process		mutually exclusive to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_30_1_183_s_140	11343654	(A) Munc13-1 and Rab3A binding to RIM1 is mutually exclusive.	bind
7002	1	2967	6	10	NULL	NULL	NULL	Munc13-1	GP		bind					RIM1	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_30_1_183_s_140	11343654	(A) Munc13-1 and Rab3A binding to RIM1 is mutually exclusive.	bind
7003	2	2967	6	10	NULL	NULL	NULL	Rab3A	GP		bind					RIM1	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_30_1_183_s_140	11343654	(A) Munc13-1 and Rab3A binding to RIM1 is mutually exclusive.	bind
7004	3	2967	6	10	NULL	NULL	NULL	statement 1	Process		is independent of					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_30_1_183_s_140	11343654	(A) Munc13-1 and Rab3A binding to RIM1 is mutually exclusive.	bind
6610	1	2968	5	10	NULL	NULL	NULL	poly-L-proline	AminoAcid		bind							mutant	Y5A		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_198	11294914	(A) Mutants that are equal to or more stable than C89S ( ) were considered as stable, including poly-L-proline binding mutants Y5A ( ), Y5D ( ), Y120D ( ), Y120A ( ), Y126D ( ) and actin binding mutants Y79R ( ), K81E ( ), K81Y ( ), P107Y (+), A111E ( ), and wild-type profilin ( ).	bind
6614	2	2968	5	10	NULL	NULL	NULL	poly-L-proline	AminoAcid		bind							mutant	Y5D		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_198	11294914	(A) Mutants that are equal to or more stable than C89S ( ) were considered as stable, including poly-L-proline binding mutants Y5A ( ), Y5D ( ), Y120D ( ), Y120A ( ), Y126D ( ) and actin binding mutants Y79R ( ), K81E ( ), K81Y ( ), P107Y (+), A111E ( ), and wild-type profilin ( ).	bind
6616	3	2968	5	10	NULL	NULL	NULL	poly-L-proline	AminoAcid		bind							mutant	Y120D		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_198	11294914	(A) Mutants that are equal to or more stable than C89S ( ) were considered as stable, including poly-L-proline binding mutants Y5A ( ), Y5D ( ), Y120D ( ), Y120A ( ), Y126D ( ) and actin binding mutants Y79R ( ), K81E ( ), K81Y ( ), P107Y (+), A111E ( ), and wild-type profilin ( ).	bind
6619	4	2968	5	10	NULL	NULL	NULL	poly-L-proline	AminoAcid		bind							mutant	Y120A		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_198	11294914	(A) Mutants that are equal to or more stable than C89S ( ) were considered as stable, including poly-L-proline binding mutants Y5A ( ), Y5D ( ), Y120D ( ), Y120A ( ), Y126D ( ) and actin binding mutants Y79R ( ), K81E ( ), K81Y ( ), P107Y (+), A111E ( ), and wild-type profilin ( ).	bind
6620	5	2968	5	10	NULL	NULL	NULL	poly-L-proline	AminoAcid		bind							mutant	Y126D		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_198	11294914	(A) Mutants that are equal to or more stable than C89S ( ) were considered as stable, including poly-L-proline binding mutants Y5A ( ), Y5D ( ), Y120D ( ), Y120A ( ), Y126D ( ) and actin binding mutants Y79R ( ), K81E ( ), K81Y ( ), P107Y (+), A111E ( ), and wild-type profilin ( ).	bind
6625	6	2968	5	10	NULL	NULL	NULL	actin	GP		bind							mutant	Y79R		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_198	11294914	(A) Mutants that are equal to or more stable than C89S ( ) were considered as stable, including poly-L-proline binding mutants Y5A ( ), Y5D ( ), Y120D ( ), Y120A ( ), Y126D ( ) and actin binding mutants Y79R ( ), K81E ( ), K81Y ( ), P107Y (+), A111E ( ), and wild-type profilin ( ).	bind
6626	7	2968	5	10	NULL	NULL	NULL	actin	GP		bind							mutant	K81E		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_198	11294914	(A) Mutants that are equal to or more stable than C89S ( ) were considered as stable, including poly-L-proline binding mutants Y5A ( ), Y5D ( ), Y120D ( ), Y120A ( ), Y126D ( ) and actin binding mutants Y79R ( ), K81E ( ), K81Y ( ), P107Y (+), A111E ( ), and wild-type profilin ( ).	bind
6627	8	2968	5	10	NULL	NULL	NULL	actin	GP		bind							mutant	K81Y		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_198	11294914	(A) Mutants that are equal to or more stable than C89S ( ) were considered as stable, including poly-L-proline binding mutants Y5A ( ), Y5D ( ), Y120D ( ), Y120A ( ), Y126D ( ) and actin binding mutants Y79R ( ), K81E ( ), K81Y ( ), P107Y (+), A111E ( ), and wild-type profilin ( ).	bind
6628	9	2968	5	10	NULL	NULL	NULL	actin	GP		bind							mutant	P107Y		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_198	11294914	(A) Mutants that are equal to or more stable than C89S ( ) were considered as stable, including poly-L-proline binding mutants Y5A ( ), Y5D ( ), Y120D ( ), Y120A ( ), Y126D ( ) and actin binding mutants Y79R ( ), K81E ( ), K81Y ( ), P107Y (+), A111E ( ), and wild-type profilin ( ).	bind
6629	10	2968	5	10	NULL	NULL	NULL	actin	GP		bind							mutant	A111E		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_198	11294914	(A) Mutants that are equal to or more stable than C89S ( ) were considered as stable, including poly-L-proline binding mutants Y5A ( ), Y5D ( ), Y120D ( ), Y120A ( ), Y126D ( ) and actin binding mutants Y79R ( ), K81E ( ), K81Y ( ), P107Y (+), A111E ( ), and wild-type profilin ( ).	bind
7005	1	2968	6	10	NULL	NULL	NULL	poly-L-proline	AminoAcid		bind							mutant	Y5A		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_198	11294914	(A) Mutants that are equal to or more stable than C89S ( ) were considered as stable, including poly-L-proline binding mutants Y5A ( ), Y5D ( ), Y120D ( ), Y120A ( ), Y126D ( ) and actin binding mutants Y79R ( ), K81E ( ), K81Y ( ), P107Y (+), A111E ( ), and wild-type profilin ( ).	bind
7006	2	2968	6	10	NULL	NULL	NULL	poly-L-proline	AminoAcid		bind							mutant	Y5D		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_198	11294914	(A) Mutants that are equal to or more stable than C89S ( ) were considered as stable, including poly-L-proline binding mutants Y5A ( ), Y5D ( ), Y120D ( ), Y120A ( ), Y126D ( ) and actin binding mutants Y79R ( ), K81E ( ), K81Y ( ), P107Y (+), A111E ( ), and wild-type profilin ( ).	bind
7007	3	2968	6	10	NULL	NULL	NULL	poly-L-proline	AminoAcid		bind							mutant	Y120A		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_198	11294914	(A) Mutants that are equal to or more stable than C89S ( ) were considered as stable, including poly-L-proline binding mutants Y5A ( ), Y5D ( ), Y120D ( ), Y120A ( ), Y126D ( ) and actin binding mutants Y79R ( ), K81E ( ), K81Y ( ), P107Y (+), A111E ( ), and wild-type profilin ( ).	bind
7008	4	2968	6	10	NULL	NULL	NULL	poly-L-proline	AminoAcid		bind							mutant	Y126D		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_198	11294914	(A) Mutants that are equal to or more stable than C89S ( ) were considered as stable, including poly-L-proline binding mutants Y5A ( ), Y5D ( ), Y120D ( ), Y120A ( ), Y126D ( ) and actin binding mutants Y79R ( ), K81E ( ), K81Y ( ), P107Y (+), A111E ( ), and wild-type profilin ( ).	bind
7009	5	2968	6	10	NULL	NULL	NULL	actin	GP		bind							mutant	Y79R		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_198	11294914	(A) Mutants that are equal to or more stable than C89S ( ) were considered as stable, including poly-L-proline binding mutants Y5A ( ), Y5D ( ), Y120D ( ), Y120A ( ), Y126D ( ) and actin binding mutants Y79R ( ), K81E ( ), K81Y ( ), P107Y (+), A111E ( ), and wild-type profilin ( ).	bind
7010	6	2968	6	10	NULL	NULL	NULL	actin	GP		bind							mutant	K81E		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_198	11294914	(A) Mutants that are equal to or more stable than C89S ( ) were considered as stable, including poly-L-proline binding mutants Y5A ( ), Y5D ( ), Y120D ( ), Y120A ( ), Y126D ( ) and actin binding mutants Y79R ( ), K81E ( ), K81Y ( ), P107Y (+), A111E ( ), and wild-type profilin ( ).	bind
7011	7	2968	6	10	NULL	NULL	NULL	actin	GP		bind							mutant	K81Y		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_198	11294914	(A) Mutants that are equal to or more stable than C89S ( ) were considered as stable, including poly-L-proline binding mutants Y5A ( ), Y5D ( ), Y120D ( ), Y120A ( ), Y126D ( ) and actin binding mutants Y79R ( ), K81E ( ), K81Y ( ), P107Y (+), A111E ( ), and wild-type profilin ( ).	bind
7012	8	2968	6	10	NULL	NULL	NULL	actin	GP		bind							mutant	P107Y (+)		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_198	11294914	(A) Mutants that are equal to or more stable than C89S ( ) were considered as stable, including poly-L-proline binding mutants Y5A ( ), Y5D ( ), Y120D ( ), Y120A ( ), Y126D ( ) and actin binding mutants Y79R ( ), K81E ( ), K81Y ( ), P107Y (+), A111E ( ), and wild-type profilin ( ).	bind
7013	9	2968	6	10	NULL	NULL	NULL	actin	GP		bind							mutant	A111E		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_198	11294914	(A) Mutants that are equal to or more stable than C89S ( ) were considered as stable, including poly-L-proline binding mutants Y5A ( ), Y5D ( ), Y120D ( ), Y120A ( ), Y126D ( ) and actin binding mutants Y79R ( ), K81E ( ), K81Y ( ), P107Y (+), A111E ( ), and wild-type profilin ( ).	bind
46577	10	2968	6	10	NULL	NULL	NULL	 poly-L-proline	AminoAcid		bind							mutant	Y120D		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_198	11294914	(A) Mutants that are equal to or more stable than C89S ( ) were considered as stable, including poly-L-proline binding mutants Y5A ( ), Y5D ( ), Y120D ( ), Y120A ( ), Y126D ( ) and actin binding mutants Y79R ( ), K81E ( ), K81Y ( ), P107Y (+), A111E ( ), and wild-type profilin ( ).	bind
6630	1	2970	5	10	NULL	NULL	NULL	PICK1	GP		bind					GluR2	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_34_1_53_s_80	11931741	(A) Mutations in the  NSF binding region  reduce PICK1 binding to GluR2.	bind
6631	2	2970	5	10	NULL	NULL	NULL			mutation in	reduce			NSF binding region		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_34_1_53_s_80	11931741	(A) Mutations in the  NSF binding region  reduce PICK1 binding to GluR2.	bind
7014	1	2970	6	10	NULL	NULL	NULL	PICK1	GP		bind					GluR2	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_34_1_53_s_80	11931741	(A) Mutations in the  NSF binding region  reduce PICK1 binding to GluR2.	bind
7015	2	2970	6	10	NULL	NULL	NULL			mutant	reduce			NSF binding region		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_34_1_53_s_80	11931741	(A) Mutations in the  NSF binding region  reduce PICK1 binding to GluR2.	bind
6632	1	2972	5	10	NULL	NULL	NULL	MutS/MutL	GP		bind					Sb-G/C-bS	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_233_s_146	12887908	(A) MutS/MutL binding to biotin-streptavidin double blocked-end G/C control DNA (Sb-G/C-bS).	bind
6633	2	2972	5	10	NULL	NULL	NULL	Sb-G/C-bS	NucleicAcid		is					biotin-streptavidin double blocked-end G/C control DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_233_s_146	12887908	(A) MutS/MutL binding to biotin-streptavidin double blocked-end G/C control DNA (Sb-G/C-bS).	bind
7016	1	2972	6	10	NULL	NULL	NULL	MutS/MutL	GP		bind					Sb-G/C-bS	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_233_s_146	12887908	(A) MutS/MutL binding to biotin-streptavidin double blocked-end G/C control DNA (Sb-G/C-bS).	bind
46578	2	2972	6	10	NULL	NULL	NULL	Sb-G/C-bS	NucleicAcid		is					 biotin-streptavidin double blocked-end G/C control DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_233_s_146	12887908	(A) MutS/MutL binding to biotin-streptavidin double blocked-end G/C control DNA (Sb-G/C-bS).	bind
6634	1	2973	5	10	NULL	NULL	NULL	NFATp	GP		bind					TNF-alpha	GP			shared sites in promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_8_2620_s_119	11909956	(A) Mutually exclusive binding of NFATp and Sp1 to shared sites in the TNF-alpha promoter.	bind
6635	2	2973	5	10	NULL	NULL	NULL	Sp1	GP		bind					TNF-alpha	GP			shared sites in promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_8_2620_s_119	11909956	(A) Mutually exclusive binding of NFATp and Sp1 to shared sites in the TNF-alpha promoter.	bind
6636	3	2973	5	10	NULL	NULL	NULL	statement 1	Process		mutually exclusive to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_8_2620_s_119	11909956	(A) Mutually exclusive binding of NFATp and Sp1 to shared sites in the TNF-alpha promoter.	bind
7017	1	2973	6	10	NULL	NULL	NULL	NFATp	GP		bind					TNF-alpha	GP			shared site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_8_2620_s_119	11909956	(A) Mutually exclusive binding of NFATp and Sp1 to shared sites in the TNF-alpha promoter.	bind
7018	2	2973	6	10	NULL	NULL	NULL	Sp1	GP		bind					TNF-alpha	GP			shared site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_8_2620_s_119	11909956	(A) Mutually exclusive binding of NFATp and Sp1 to shared sites in the TNF-alpha promoter.	bind
7019	3	2973	6	10	NULL	NULL	NULL	statement 1	Process		is mutually exclusive to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_8_2620_s_119	11909956	(A) Mutually exclusive binding of NFATp and Sp1 to shared sites in the TNF-alpha promoter.	bind
6637	1	2974	5	10	NULL	NULL	NULL	VDR	GP		bind					GM550	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4191_s_138	10330159	(A) Mutually exclusive binding of VDR and NFATXS to GM550.	bind
6638	2	2974	5	10	NULL	NULL	NULL	NFATXS	GP		bind					GM550	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4191_s_138	10330159	(A) Mutually exclusive binding of VDR and NFATXS to GM550.	bind
6639	3	2974	5	10	NULL	NULL	NULL	statement 1	Process		mutually exclusive to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4191_s_138	10330159	(A) Mutually exclusive binding of VDR and NFATXS to GM550.	bind
7028	1	2974	6	10	NULL	NULL	NULL	VDR	GP		bind					GM550	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4191_s_138	10330159	(A) Mutually exclusive binding of VDR and NFATXS to GM550.	bind
7029	2	2974	6	10	NULL	NULL	NULL	NFATXS	GP		bind					GM550	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4191_s_138	10330159	(A) Mutually exclusive binding of VDR and NFATXS to GM550.	bind
7030	3	2974	6	10	NULL	NULL	NULL	statement 1	Process		is mutually exclusive to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4191_s_138	10330159	(A) Mutually exclusive binding of VDR and NFATXS to GM550.	bind
6640	1	2975	5	10	NULL	NULL	NULL				bind			 N1-47		NusA	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_265_s_114	9659923	(A) N1-47 binds NusA.	bind
7031	1	2975	6	10	NULL	NULL	NULL				bind			N1-47		NusA	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_265_s_114	9659923	(A) N1-47 binds NusA.	bind
6641	1	2976	5	10	NULL	NULL	NULL	N2N	GP		bind		directly			NE	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_1_58_s_196	14673143	(A) N2N directly binds  to NE in GST pull-down assays.	bind
7032	1	2976	6	10	NULL	NULL	NULL	N2N	GP		bind		directly			NE	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_1_58_s_196	14673143	(A) N2N directly binds  to NE in GST pull-down assays.	bind
6642	1	2977	5	10	NULL	NULL	NULL	NC2alpha	GP		bind					DNA	NucleicAcid			B-TFIID	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_22_10072_s_225	15509807	(A) NC2alpha binds to both B-TFIID and TBP on DNA.	bind
6643	2	2977	5	10	NULL	NULL	NULL	NC2alpha	GP		bind					DNA	NucleicAcid			TBP	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_22_10072_s_225	15509807	(A) NC2alpha binds to both B-TFIID and TBP on DNA.	bind
7033	1	2977	6	10	NULL	NULL	NULL	NC2alpha	GP		bind					DNA	NucleicAcid			B-TFIID site	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_22_10072_s_225	15509807	(A) NC2alpha binds to both B-TFIID and TBP on DNA.	bind
7034	2	2977	6	10	NULL	NULL	NULL	NC2alpha	GP		bind					DNA	NucleicAcid			TBP site	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_22_10072_s_225	15509807	(A) NC2alpha binds to both B-TFIID and TBP on DNA.	bind
6644	1	2978	5	10	NULL	NULL	NULL	Nck	GP		bind					CD3	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_109_7_901_s_41	12110186	(A) Nck binds to CD3  but not to other CD3 subunits.	bind
6645	2	2978	5	10	NULL	NULL	NULL	Nck	GP		does not bind					CD3	GP		other subunits of		NULL		NULL	NULL	NULL	NULL	gw60_cell_109_7_901_s_41	12110186	(A) Nck binds to CD3  but not to other CD3 subunits.	bind
7035	1	2978	6	10	NULL	NULL	NULL	Nck	GP		bind					CD3	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_109_7_901_s_41	12110186	(A) Nck binds to CD3  but not to other CD3 subunits.	bind
7036	2	2978	6	10	NULL	NULL	NULL	Nck	GP		does not bind					CD3 	GP		subunits		NULL		NULL	NULL	NULL	NULL	gw60_cell_109_7_901_s_41	12110186	(A) Nck binds to CD3  but not to other CD3 subunits.	bind
6646	1	2979	5	10	NULL	NULL	NULL	NE proteins	GP		bind					A3 RNA	NucleicAcid	biotinylated			NULL		NULL	NULL	NULL	NULL	gw60_cell_93_1_139_s_84	9546399	(A) NE proteins  bound to biotinylated A3 or S3 RNA were analyzed by Western blot  with anti-Tra2 antibodies (lanes 1 - 4) or mAb104 (lanes 5 - 8) before (-) or after (+) treatment with  CIP.	bind
6647	2	2979	5	10	NULL	NULL	NULL	NE proteins	GP		bind					S3 RNA	NucleicAcid	biotinylated			NULL		NULL	NULL	NULL	NULL	gw60_cell_93_1_139_s_84	9546399	(A) NE proteins  bound to biotinylated A3 or S3 RNA were analyzed by Western blot  with anti-Tra2 antibodies (lanes 1 - 4) or mAb104 (lanes 5 - 8) before (-) or after (+) treatment with  CIP.	bind
46580	3	2979	5	10	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_93_1_139_s_84	9546399	(A) NE proteins  bound to biotinylated A3 or S3 RNA were analyzed by Western blot  with anti-Tra2 antibodies (lanes 1 - 4) or mAb104 (lanes 5 - 8) before (-) or after (+) treatment with  CIP.	bind
7037	1	2979	6	10	NULL	NULL	NULL	NE proteins	GP		bind					A3 RNA	NucleicAcid	biotinylated			NULL		NULL	NULL	NULL	NULL	gw60_cell_93_1_139_s_84	9546399	(A) NE proteins  bound to biotinylated A3 or S3 RNA were analyzed by Western blot  with anti-Tra2 antibodies (lanes 1 - 4) or mAb104 (lanes 5 - 8) before (-) or after (+) treatment with  CIP.	bind
7038	2	2979	6	10	NULL	NULL	NULL	NE proteins	GP		bind					S3 RNA	NucleicAcid	biotinylated			NULL		NULL	NULL	NULL	NULL	gw60_cell_93_1_139_s_84	9546399	(A) NE proteins  bound to biotinylated A3 or S3 RNA were analyzed by Western blot  with anti-Tra2 antibodies (lanes 1 - 4) or mAb104 (lanes 5 - 8) before (-) or after (+) treatment with  CIP.	bind
7039	3	2979	6	10	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_93_1_139_s_84	9546399	(A) NE proteins  bound to biotinylated A3 or S3 RNA were analyzed by Western blot  with anti-Tra2 antibodies (lanes 1 - 4) or mAb104 (lanes 5 - 8) before (-) or after (+) treatment with  CIP.	bind
6648	1	2980	5	10	NULL	NULL	NULL	Nef	GP		bind					MHC-I	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_70_2_548_s_178	16760313	(A) Nef binds to MHC-I  early in the secretory pathway.	bind
6649	2	2980	5	10	NULL	NULL	NULL	statement 1	Process		occur					secretory pathway	Process	early in 			NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_70_2_548_s_178	16760313	(A) Nef binds to MHC-I  early in the secretory pathway.	bind
7040	1	2980	6	10	NULL	NULL	NULL	Nef	GP		bind					MHC-I	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_70_2_548_s_178	16760313	(A) Nef binds to MHC-I  early in the secretory pathway.	bind
7041	2	2980	6	10	NULL	NULL	NULL	statement 1	Process		occurs 					secretory pathway	Process	early in			NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_70_2_548_s_178	16760313	(A) Nef binds to MHC-I  early in the secretory pathway.	bind
6650	1	2981	5	10	NULL	NULL	NULL	Smc2p	GP		bind					chromosome VI	Chromosome			replication origins	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7216_s_120	16055730	(A) Negative  correlation between Smc2p and ORC complex binding at chromosome (Chr.) VI replication  origins.	bind
6651	2	2981	5	10	NULL	NULL	NULL	ORC complex	GP		bind					chromosome  VI	Chromosome			replication origins	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7216_s_120	16055730	(A) Negative  correlation between Smc2p and ORC complex binding at chromosome (Chr.) VI replication  origins.	bind
7042	1	2981	6	10	NULL	NULL	NULL	Smc2p	GP		bind					chromosome VI 	Chromosome			replication origins	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7216_s_120	16055730	(A) Negative  correlation between Smc2p and ORC complex binding at chromosome (Chr.) VI replication  origins.	bind
7043	2	2981	6	10	NULL	NULL	NULL	ORC complex	GP		bind					chromosome VI 	Chromosome			replication origins	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7216_s_120	16055730	(A) Negative  correlation between Smc2p and ORC complex binding at chromosome (Chr.) VI replication  origins.	bind
6652	1	2982	5	10	NULL	NULL	NULL	LDL	Chemical		bind		specifically			mSR-AI	GP				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_4_753_s_105	10191300	(A) Net specific binding activity of LDL to mSR-AI mediated by peptide V.	bind
6653	2	2982	5	10	NULL	NULL	NULL	statement 1	Process		is mediated by					peptide V	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_4_753_s_105	10191300	(A) Net specific binding activity of LDL to mSR-AI mediated by peptide V.	bind
7044	1	2982	6	10	NULL	NULL	NULL	LDL	Chemical		bind		specifically			mSR-AI	GP				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_4_753_s_105	10191300	(A) Net specific binding activity of LDL to mSR-AI mediated by peptide V.	bind
7045	2	2982	6	10	NULL	NULL	NULL	statement 1	Process		is mediated by					peptide V	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_4_753_s_105	10191300	(A) Net specific binding activity of LDL to mSR-AI mediated by peptide V.	bind
7135	1	2983	5	10	NULL	NULL	NULL	CTX	GP		bind		specifically			GM1	Chemical				NULL	Neuro2a cells	NULL	NULL	NULL	NULL	gw60_cellbiol_159_1_157_s_161	12370242	(A) Neuro2a cells transfected with a GFRalpha1 construct were Triton-extracted and fixed with 4% PFA before staining with an antibody to GFRalpha1 and cholera toxin (CTX), which specifically binds to the lipid raft ganglioside GM1.	bind
7136	2	2983	5	10	NULL	NULL	NULL	CTX	GP		is					cholera toxin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_1_157_s_161	12370242	(A) Neuro2a cells transfected with a GFRalpha1 construct were Triton-extracted and fixed with 4% PFA before staining with an antibody to GFRalpha1 and cholera toxin (CTX), which specifically binds to the lipid raft ganglioside GM1.	bind
7137	3	2983	5	10	NULL	NULL	NULL	GFRalpha1	GP		bind		specifically			GM1	Chemical				NULL	Neuro2a cells	NULL	NULL	NULL	NULL	gw60_cellbiol_159_1_157_s_161	12370242	(A) Neuro2a cells transfected with a GFRalpha1 construct were Triton-extracted and fixed with 4% PFA before staining with an antibody to GFRalpha1 and cholera toxin (CTX), which specifically binds to the lipid raft ganglioside GM1.	bind
46584	4	2983	5	10	NULL	NULL	NULL	GM1	Chemical		is a type of					lipid raft ganglioside	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_1_157_s_161	12370242	(A) Neuro2a cells transfected with a GFRalpha1 construct were Triton-extracted and fixed with 4% PFA before staining with an antibody to GFRalpha1 and cholera toxin (CTX), which specifically binds to the lipid raft ganglioside GM1.	bind
7046	1	2983	6	10	NULL	NULL	NULL	GM1	Chemical		is a type of					lipid raft ganglioside	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_1_157_s_161	12370242	(A) Neuro2a cells transfected with a GFRalpha1 construct were Triton-extracted and fixed with 4% PFA before staining with an antibody to GFRalpha1 and cholera toxin (CTX), which specifically binds to the lipid raft ganglioside GM1.	bind
7047	2	2983	6	10	NULL	NULL	NULL	GFRalpha1	GP		bind		specifically			GM1	Chemical				NULL	Neuro2a cells	NULL	NULL	NULL	NULL	gw60_cellbiol_159_1_157_s_161	12370242	(A) Neuro2a cells transfected with a GFRalpha1 construct were Triton-extracted and fixed with 4% PFA before staining with an antibody to GFRalpha1 and cholera toxin (CTX), which specifically binds to the lipid raft ganglioside GM1.	bind
7048	3	2983	6	10	NULL	NULL	NULL	Cholera toxin	GP		bind		specifically			GM1	Chemical				NULL	Neuro2a cells	NULL	NULL	NULL	NULL	gw60_cellbiol_159_1_157_s_161	12370242	(A) Neuro2a cells transfected with a GFRalpha1 construct were Triton-extracted and fixed with 4% PFA before staining with an antibody to GFRalpha1 and cholera toxin (CTX), which specifically binds to the lipid raft ganglioside GM1.	bind
7049	4	2983	6	10	NULL	NULL	NULL	CTX	GP		is					cholera toxin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_1_157_s_161	12370242	(A) Neuro2a cells transfected with a GFRalpha1 construct were Triton-extracted and fixed with 4% PFA before staining with an antibody to GFRalpha1 and cholera toxin (CTX), which specifically binds to the lipid raft ganglioside GM1.	bind
6654	1	2986	5	10	NULL	NULL	NULL	NG2	GP		bind					EC surface	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_8_3580_s_128	15181153	(A) NG2 binding to the EC surface.	bind
7050	1	2986	6	10	NULL	NULL	NULL	NG2	GP		bind					EC surface	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_8_3580_s_128	15181153	(A) NG2 binding to the EC surface.	bind
6655	1	2987	5	10	NULL	NULL	NULL	VCAM-1	GP	soluble	bind					T cells	Cell	activated			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_3_509_s_107	11980922	(A) NH2-terminal regions of TSP1 and TSP2 inhibit binding of soluble VCAM-1 to activated T cells.	bind
6656	2	2987	5	10	NULL	NULL	NULL	TSP1	GP		inhibit			NH2-terminal region		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_3_509_s_107	11980922	(A) NH2-terminal regions of TSP1 and TSP2 inhibit binding of soluble VCAM-1 to activated T cells.	bind
6657	3	2987	5	10	NULL	NULL	NULL	TSP2	GP		inhibit			NH2-terminal region		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_3_509_s_107	11980922	(A) NH2-terminal regions of TSP1 and TSP2 inhibit binding of soluble VCAM-1 to activated T cells.	bind
7051	1	2987	6	10	NULL	NULL	NULL	VCAM-1	GP	soluble	bind					T cells	Cell	activated			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_3_509_s_107	11980922	(A) NH2-terminal regions of TSP1 and TSP2 inhibit binding of soluble VCAM-1 to activated T cells.	bind
7052	2	2987	6	10	NULL	NULL	NULL	TSP1	GP		inhibit			NH2-terminus		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_3_509_s_107	11980922	(A) NH2-terminal regions of TSP1 and TSP2 inhibit binding of soluble VCAM-1 to activated T cells.	bind
7053	3	2987	6	10	NULL	NULL	NULL	TSP2	GP		inhibit			NH2-terminus		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_3_509_s_107	11980922	(A) NH2-terminal regions of TSP1 and TSP2 inhibit binding of soluble VCAM-1 to activated T cells.	bind
6658	1	2989	5	10	NULL	NULL	NULL	LdTOP1L	GP		bind					LdTOP1S	GP				NULL		NULL	NULL	NULL	NULL	gw70_febslett_565_1_81_s_184	15135057	(A) Ni2+-NTA agarose co-immobilization binding between LdTOP1L and LdTOP1S.	bind
7054	1	2989	6	10	NULL	NULL	NULL	LdTOP1L	GP		bind					LdTOP1S	GP				NULL		NULL	NULL	NULL	NULL	gw70_febslett_565_1_81_s_184	15135057	(A) Ni2+-NTA agarose co-immobilization binding between LdTOP1L and LdTOP1S.	bind
7138	1	2991	5	10	NULL	NULL	NULL				mediate			NLS		NRK cells	Cell	import in			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_2_411_s_119	11266456	(A) NLS-mediated import in NRK cells; (B) the solubilization of Nup358 and Nup153 (left) and the association of importin beta with these Nups (right); and (C) the binding of importin beta to GST-Nup62.	bind
7141	4	2991	5	10	NULL	NULL	NULL	importin beta	GP		associate with					Nup358	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_2_411_s_119	11266456	(A) NLS-mediated import in NRK cells; (B) the solubilization of Nup358 and Nup153 (left) and the association of importin beta with these Nups (right); and (C) the binding of importin beta to GST-Nup62.	bind
7142	5	2991	5	10	NULL	NULL	NULL	importin beta	GP		associate with					Nup153	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_2_411_s_119	11266456	(A) NLS-mediated import in NRK cells; (B) the solubilization of Nup358 and Nup153 (left) and the association of importin beta with these Nups (right); and (C) the binding of importin beta to GST-Nup62.	bind
7143	6	2991	5	10	NULL	NULL	NULL	importin beta	GP		bind					GST-Nup62	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_2_411_s_119	11266456	(A) NLS-mediated import in NRK cells; (B) the solubilization of Nup358 and Nup153 (left) and the association of importin beta with these Nups (right); and (C) the binding of importin beta to GST-Nup62.	bind
7251	1	2991	6	10	NULL	NULL	NULL				mediates			NLS		NRK cells	Cell	import in			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_2_411_s_119	11266456	(A) NLS-mediated import in NRK cells; (B) the solubilization of Nup358 and Nup153 (left) and the association of importin beta with these Nups (right); and (C) the binding of importin beta to GST-Nup62.	bind
7252	2	2991	6	10	NULL	NULL	NULL	importin beta	GP		associates					Nup358	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_2_411_s_119	11266456	(A) NLS-mediated import in NRK cells; (B) the solubilization of Nup358 and Nup153 (left) and the association of importin beta with these Nups (right); and (C) the binding of importin beta to GST-Nup62.	bind
7253	3	2991	6	10	NULL	NULL	NULL	importin beta	GP		associates					Nup153	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_2_411_s_119	11266456	(A) NLS-mediated import in NRK cells; (B) the solubilization of Nup358 and Nup153 (left) and the association of importin beta with these Nups (right); and (C) the binding of importin beta to GST-Nup62.	bind
7254	4	2991	6	10	NULL	NULL	NULL	importin beta	GP		bind					GST-Nup62	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_2_411_s_119	11266456	(A) NLS-mediated import in NRK cells; (B) the solubilization of Nup358 and Nup153 (left) and the association of importin beta with these Nups (right); and (C) the binding of importin beta to GST-Nup62.	bind
6659	2	2992	5	10	NULL	NULL	NULL	Nmd3p	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_10_3405_s_187	11313466	(A) Nmd3p binds to GST-tagged Rpl10p when expressed in  E. coli.	bind
53116	1	2992	5	10	NULL	NULL	NULL	Rpl10p	GP	GST-tagged	is expressed in					E.coli	Cell				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_10_3405_s_187	11313466	(A) Nmd3p binds to GST-tagged Rpl10p when expressed in  E. coli.	bind
7055	1	2992	6	10	NULL	NULL	NULL	Rpl10p	GP	GST-tagged	expressed in					E.coli	Cell				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_10_3405_s_187	11313466	(A) Nmd3p binds to GST-tagged Rpl10p when expressed in  E. coli.	bind
7056	2	2992	6	10	NULL	NULL	NULL	Nmd3p	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_10_3405_s_187	11313466	(A) Nmd3p binds to GST-tagged Rpl10p when expressed in  E. coli.	bind
6660	1	2993	5	10	NULL	NULL	NULL	Nmd5p	GP		bind					GST - Crz1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_951_s_108	11535618	(A) Nmd5p binding to Crz1p is disrupted by Gsp1p - GTP. 5 mug GST - Crz1p was bound to glutathione resin and incubated with 5 mug thrombin-cleaved Nmd5p.	bind
6661	2	2993	5	10	NULL	NULL	NULL	Gsp1p - GTP	GP		disrupt					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_951_s_108	11535618	(A) Nmd5p binding to Crz1p is disrupted by Gsp1p - GTP. 5 mug GST - Crz1p was bound to glutathione resin and incubated with 5 mug thrombin-cleaved Nmd5p.	bind
7057	1	2993	6	10	NULL	NULL	NULL	Nmd5p	GP		bind					GST - Crz1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_951_s_108	11535618	(A) Nmd5p binding to Crz1p is disrupted by Gsp1p - GTP. 5 mug GST - Crz1p was bound to glutathione resin and incubated with 5 mug thrombin-cleaved Nmd5p.	bind
7058	2	2993	6	10	NULL	NULL	NULL	Gsp1p - GTP	GP		disrupts					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_951_s_108	11535618	(A) Nmd5p binding to Crz1p is disrupted by Gsp1p - GTP. 5 mug GST - Crz1p was bound to glutathione resin and incubated with 5 mug thrombin-cleaved Nmd5p.	bind
6663	1	2994	5	10	NULL	NULL	NULL	Nocodazole	Chemical		does not depolymerize					CPP MTs	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_161_2_349_s_160	12719474	(A) Nocodazole does not depolymerize CPP MTs in our assay.	bind
7059	1	2994	6	10	NULL	NULL	NULL	Nocodazole	Chemical		does not depolymerize					CPP MTs	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_161_2_349_s_160	12719474	(A) Nocodazole does not depolymerize CPP MTs in our assay.	bind
7144	1	2995	5	10	NULL	NULL	NULL	M21 cell extracts 		normoxic	bind					HSR probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_2_469_s_219	9450968	(A) Normoxic (N) and hypoxic (H) M21 cell extracts bound to the 3  HSR probe were subjected to UV-cross-linking/Nase treatment and analyzed by reducing SDS-PAGE.	bind
7145	2	2995	5	10	NULL	NULL	NULL	M21 cell extracts		hypoxic	bind					HSR probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_2_469_s_219	9450968	(A) Normoxic (N) and hypoxic (H) M21 cell extracts bound to the 3  HSR probe were subjected to UV-cross-linking/Nase treatment and analyzed by reducing SDS-PAGE.	bind
7060	1	2995	6	10	NULL	NULL	NULL	M21 cell extracts		Normoxic	bind					HSR probe	NucleicAcid			site	NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_2_469_s_219	9450968	(A) Normoxic (N) and hypoxic (H) M21 cell extracts bound to the 3  HSR probe were subjected to UV-cross-linking/Nase treatment and analyzed by reducing SDS-PAGE.	bind
7061	2	2995	6	10	NULL	NULL	NULL	M21 cell extracts		hypoxic	bind					HSR probe	NucleicAcid			site	NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_2_469_s_219	9450968	(A) Normoxic (N) and hypoxic (H) M21 cell extracts bound to the 3  HSR probe were subjected to UV-cross-linking/Nase treatment and analyzed by reducing SDS-PAGE.	bind
6665	1	2996	5	10	NULL	NULL	NULL	[35]GTP S 	Chemical		bind					MBP-T43NTR-G 	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_493_2_101_s_100	11287004	(A) NT-induced [35]GTP S binding to  E. coli membrane-inserted MBP-T43NTR-G  fusion proteins or to homogenates of transfected CHO-NTR cells expressing the rat NTR.	bind
6666	2	2996	5	10	NULL	NULL	NULL	NT	GP		induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_493_2_101_s_100	11287004	(A) NT-induced [35]GTP S binding to  E. coli membrane-inserted MBP-T43NTR-G  fusion proteins or to homogenates of transfected CHO-NTR cells expressing the rat NTR.	bind
6667	3	2996	5	10	NULL	NULL	NULL	CHO-NTR cells	Cell	homogenates of transfected	express					NTR	GP	rat			NULL		NULL	NULL	NULL	NULL	gw60_febslett_493_2_101_s_100	11287004	(A) NT-induced [35]GTP S binding to  E. coli membrane-inserted MBP-T43NTR-G  fusion proteins or to homogenates of transfected CHO-NTR cells expressing the rat NTR.	bind
6668	4	2996	5	10	NULL	NULL	NULL	[35]GTP S	Chemical		bind					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_493_2_101_s_100	11287004	(A) NT-induced [35]GTP S binding to  E. coli membrane-inserted MBP-T43NTR-G  fusion proteins or to homogenates of transfected CHO-NTR cells expressing the rat NTR.	bind
6669	5	2996	5	10	NULL	NULL	NULL	NT	GP		induce					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_493_2_101_s_100	11287004	(A) NT-induced [35]GTP S binding to  E. coli membrane-inserted MBP-T43NTR-G  fusion proteins or to homogenates of transfected CHO-NTR cells expressing the rat NTR.	bind
53125	6	2996	5	10	NULL	NULL	NULL	MBP-T43NTR-G	GP		is a type of					fusion protein	GP	E. coli membrane-inserted			NULL		NULL	NULL	NULL	NULL	gw60_febslett_493_2_101_s_100	11287004	(A) NT-induced [35]GTP S binding to  E. coli membrane-inserted MBP-T43NTR-G  fusion proteins or to homogenates of transfected CHO-NTR cells expressing the rat NTR.	bind
7255	1	2996	6	10	NULL	NULL	NULL	[35]GTP S	Chemical		bind					MBP-T43NTR-G 	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_493_2_101_s_100	11287004	(A) NT-induced [35]GTP S binding to  E. coli membrane-inserted MBP-T43NTR-G  fusion proteins or to homogenates of transfected CHO-NTR cells expressing the rat NTR.	bind
7256	2	2996	6	10	NULL	NULL	NULL	NT	GP		induces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_493_2_101_s_100	11287004	(A) NT-induced [35]GTP S binding to  E. coli membrane-inserted MBP-T43NTR-G  fusion proteins or to homogenates of transfected CHO-NTR cells expressing the rat NTR.	bind
7279	3	2996	6	10	NULL	NULL	NULL	CHO-NTR cells 	Cell		express					NTR	GP	rat			NULL		NULL	NULL	NULL	NULL	gw60_febslett_493_2_101_s_100	11287004	(A) NT-induced [35]GTP S binding to  E. coli membrane-inserted MBP-T43NTR-G  fusion proteins or to homogenates of transfected CHO-NTR cells expressing the rat NTR.	bind
7280	4	2996	6	10	NULL	NULL	NULL	GTP S	Chemical		bind					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_493_2_101_s_100	11287004	(A) NT-induced [35]GTP S binding to  E. coli membrane-inserted MBP-T43NTR-G  fusion proteins or to homogenates of transfected CHO-NTR cells expressing the rat NTR.	bind
46585	5	2996	6	10	NULL	NULL	NULL	NT	GP		induce					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_493_2_101_s_100	11287004	(A) NT-induced [35]GTP S binding to  E. coli membrane-inserted MBP-T43NTR-G  fusion proteins or to homogenates of transfected CHO-NTR cells expressing the rat NTR.	bind
53126	6	2996	6	10	NULL	NULL	NULL	MBP-T43NTR-G	GP		is a type of					fusion protein	GP	E. coli membrane-inserted			NULL		NULL	NULL	NULL	NULL	gw60_febslett_493_2_101_s_100	11287004	(A) NT-induced [35]GTP S binding to  E. coli membrane-inserted MBP-T43NTR-G  fusion proteins or to homogenates of transfected CHO-NTR cells expressing the rat NTR.	bind
6664	1	3001	5	10	NULL	NULL	NULL	Nup60p	GP		bind					Gsp1p - GTP	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_937_s_176	11535617	(A) Nup60p binds Gsp1p - GTP.	bind
7062	1	3001	6	10	NULL	NULL	NULL	Nup60p	GP		bind					Gsp1p - GTP	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_937_s_176	11535617	(A) Nup60p binds Gsp1p - GTP.	bind
6670	1	3002	5	10	NULL	NULL	NULL	Nup60p	GP		bind					Kap95p	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_937_s_65	11535617	(A) Nup60p binds Kap95p, but only in the absence of Gsp1p - GTP.	bind
6671	2	3002	5	10	NULL	NULL	NULL	statement 1	Process		occurs in absence of		only			Gsp1p - GTP	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_937_s_65	11535617	(A) Nup60p binds Kap95p, but only in the absence of Gsp1p - GTP.	bind
7063	1	3002	6	10	NULL	NULL	NULL	Nup60p	GP		bind					Kap95p	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_937_s_65	11535617	(A) Nup60p binds Kap95p, but only in the absence of Gsp1p - GTP.	bind
7064	2	3002	6	10	NULL	NULL	NULL	statement 1	Process		occurs in absence of		only			Gsp1p - GTP	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_937_s_65	11535617	(A) Nup60p binds Kap95p, but only in the absence of Gsp1p - GTP.	bind
6672	1	3003	5	10	NULL	NULL	NULL	NURF	GP		bind					HSF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_3_531_s_194	11583616	(A) NURF binds to HSF and VP16.	bind
6673	2	3003	5	10	NULL	NULL	NULL	NURF	GP		bind					VP16	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_3_531_s_194	11583616	(A) NURF binds to HSF and VP16.	bind
7065	1	3003	6	10	NULL	NULL	NULL	NURF	GP		bind					HSF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_3_531_s_194	11583616	(A) NURF binds to HSF and VP16.	bind
7066	2	3003	6	10	NULL	NULL	NULL	NURF	GP		bind					VP16	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_3_531_s_194	11583616	(A) NURF binds to HSF and VP16.	bind
6674	1	3004	5	10	NULL	NULL	NULL	Oct-1 	GP		bind					HLA-DRA 	GP			octamer element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6495_s_283	11533238	(A) Oct-1 binding to the HLA-DRA octamer element is disrupted by HDAC inhibitors.	bind
6675	2	3004	5	10	NULL	NULL	NULL	HDAC inhibitors	Chemical		disrupt					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6495_s_283	11533238	(A) Oct-1 binding to the HLA-DRA octamer element is disrupted by HDAC inhibitors.	bind
7174	1	3004	6	10	NULL	NULL	NULL	Oct-1	GP		bind					HLA-DRA	GP			octamer element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6495_s_283	11533238	(A) Oct-1 binding to the HLA-DRA octamer element is disrupted by HDAC inhibitors.	bind
7175	2	3004	6	10	NULL	NULL	NULL	HDAC inhibitors	Chemical		disrupts					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6495_s_283	11533238	(A) Oct-1 binding to the HLA-DRA octamer element is disrupted by HDAC inhibitors.	bind
6676	1	3005	5	10	NULL	NULL	NULL	Bcd	GP		bind					TAF60	GP				NULL		NULL	NULL	NULL	NULL	gw60_development_128_12_2281_s_223	11493547	(A) of Bcd binds TAF60, this type of domain is also frequently implicated in transcriptional repression in vivo ( Hanna-Rose and Hansen, 1996).	bind
7177	1	3005	6	10	NULL	NULL	NULL	Bcd	GP		bind					TAF60	GP				NULL		NULL	NULL	NULL	NULL	gw60_development_128_12_2281_s_223	11493547	(A) of Bcd binds TAF60, this type of domain is also frequently implicated in transcriptional repression in vivo ( Hanna-Rose and Hansen, 1996).	bind
6677	1	3006	5	10	NULL	NULL	NULL				bind			tail		PAB	GP	endogenous			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_17_4723_s_259	10970864	(A) on the reporter mRNAs in yeast cells; the tails could bind endogenous PAB and minimize MS2 - yPAB s effects.	bind
6678	2	3006	5	10	NULL	NULL	NULL	statement 1	Process		minimize					MS2 - yPAB s effects	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_17_4723_s_259	10970864	(A) on the reporter mRNAs in yeast cells; the tails could bind endogenous PAB and minimize MS2 - yPAB s effects.	bind
7178	1	3006	6	10	NULL	NULL	NULL				bind			tails		PAB	GP	endogenous			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_17_4723_s_259	10970864	(A) on the reporter mRNAs in yeast cells; the tails could bind endogenous PAB and minimize MS2 - yPAB s effects.	bind
7179	2	3006	6	10	NULL	NULL	NULL	statement 1	Process		minimize					MS2 - yPAB s effects	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_17_4723_s_259	10970864	(A) on the reporter mRNAs in yeast cells; the tails could bind endogenous PAB and minimize MS2 - yPAB s effects.	bind
6679	1	3007	5	10	NULL	NULL	NULL	E2BD	AminoAcid		bind					E3 dimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_structure_4_3_277_s_109	8805537	(a) One E2BD (blue) is shown bound to one E3 dimer, as observed in the crystal structure.	bind
7180	1	3007	6	10	NULL	NULL	NULL	E2BD	AminoAcid		bind					E3 dimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_structure_4_3_277_s_109	8805537	(a) One E2BD (blue) is shown bound to one E3 dimer, as observed in the crystal structure.	bind
6681	1	3016	5	10	NULL	NULL	NULL	Pc	GP	oxidized	bind					EYL:DOTAP+	Chemical				NULL	large unilamellar vesicles	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1463_2_429_s_69	10675519	(A) Original infrared spectra corresponding to oxidized Pc bound to EYL:DOTAP+ (1:4 molar ratio) large unilamellar vesicles (----), and to the same liposome suspension in the absence of protein (- - -).	bind
7182	1	3016	6	10	NULL	NULL	NULL	Pc	GP	oxidized	bind					EYL:DOTAP+	Chemical				NULL	large unilamellar vesicles	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1463_2_429_s_69	10675519	(A) Original infrared spectra corresponding to oxidized Pc bound to EYL:DOTAP+ (1:4 molar ratio) large unilamellar vesicles (----), and to the same liposome suspension in the absence of protein (- - -).	bind
6682	1	3017	5	10	NULL	NULL	NULL	Munc18c	GP	overexpression of	occludes								syntaxin 4 binding sites		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_1_379_s_266	10594040	(A) Overexpression of Munc18c occludes all the syntaxin 4 binding sites, thereby preventing the association of the GSV with the plasma membrane and hence translocation.	bind
6683	2	3017	5	10	NULL	NULL	NULL	GSV	CellComponent		associate with					plasma membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_1_379_s_266	10594040	(A) Overexpression of Munc18c occludes all the syntaxin 4 binding sites, thereby preventing the association of the GSV with the plasma membrane and hence translocation.	bind
6684	3	3017	5	10	NULL	NULL	NULL	statement 1	Process		prevent					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_1_379_s_266	10594040	(A) Overexpression of Munc18c occludes all the syntaxin 4 binding sites, thereby preventing the association of the GSV with the plasma membrane and hence translocation.	bind
6685	4	3017	5	10	NULL	NULL	NULL	statement 1	Process		prevents					GSV	CellComponent	translocation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_1_379_s_266	10594040	(A) Overexpression of Munc18c occludes all the syntaxin 4 binding sites, thereby preventing the association of the GSV with the plasma membrane and hence translocation.	bind
7257	1	3017	6	10	NULL	NULL	NULL	GSV	CellComponent		associates					plasma membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_1_379_s_266	10594040	(A) Overexpression of Munc18c occludes all the syntaxin 4 binding sites, thereby preventing the association of the GSV with the plasma membrane and hence translocation.	bind
7258	2	3017	6	10	NULL	NULL	NULL	Munc18c	GP	overexpression	occludes								syntaxin 4 binding site		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_1_379_s_266	10594040	(A) Overexpression of Munc18c occludes all the syntaxin 4 binding sites, thereby preventing the association of the GSV with the plasma membrane and hence translocation.	bind
7259	3	3017	6	10	NULL	NULL	NULL	statement 2	Process		prevents					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_1_379_s_266	10594040	(A) Overexpression of Munc18c occludes all the syntaxin 4 binding sites, thereby preventing the association of the GSV with the plasma membrane and hence translocation.	bind
7260	4	3017	6	10	NULL	NULL	NULL	statement 2	Process		prevents					GSV	CellComponent	translocation of 			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_1_379_s_266	10594040	(A) Overexpression of Munc18c occludes all the syntaxin 4 binding sites, thereby preventing the association of the GSV with the plasma membrane and hence translocation.	bind
6686	1	3018	5	10	NULL	NULL	NULL	p35	GP		bind					GST-hAATYKs-p35BPN169	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_310_2_398_s_95	14521924	(A) p35 or Cdk5 bound  to GST-hAATYKs-p35BPN169 (lanes 1-3) was detected by immunoblotting with anti-p35 (p35) or anti-Cdk5 (Cdk5).	bind
6687	2	3018	5	10	NULL	NULL	NULL	Cdk5	GP		bind					GST-hAATYKs-p35BPN169	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_310_2_398_s_95	14521924	(A) p35 or Cdk5 bound  to GST-hAATYKs-p35BPN169 (lanes 1-3) was detected by immunoblotting with anti-p35 (p35) or anti-Cdk5 (Cdk5).	bind
53128	3	3018	5	10	NULL	NULL	NULL	statement 1	GP		is an alternative to					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_310_2_398_s_95	14521924	(A) p35 or Cdk5 bound  to GST-hAATYKs-p35BPN169 (lanes 1-3) was detected by immunoblotting with anti-p35 (p35) or anti-Cdk5 (Cdk5).	bind
7183	1	3018	6	10	NULL	NULL	NULL	p35	GP		bind					GST-hAATYKs-p35BPN169	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_310_2_398_s_95	14521924	(A) p35 or Cdk5 bound  to GST-hAATYKs-p35BPN169 (lanes 1-3) was detected by immunoblotting with anti-p35 (p35) or anti-Cdk5 (Cdk5).	bind
7184	2	3018	6	10	NULL	NULL	NULL	Cdk5	GP		bind					GST-hAATYKs-p35BPN169	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_310_2_398_s_95	14521924	(A) p35 or Cdk5 bound  to GST-hAATYKs-p35BPN169 (lanes 1-3) was detected by immunoblotting with anti-p35 (p35) or anti-Cdk5 (Cdk5).	bind
7185	3	3018	6	10	NULL	NULL	NULL	statement 1	GP		is an alternative to					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_310_2_398_s_95	14521924	(A) p35 or Cdk5 bound  to GST-hAATYKs-p35BPN169 (lanes 1-3) was detected by immunoblotting with anti-p35 (p35) or anti-Cdk5 (Cdk5).	bind
6688	1	3019	5	10	NULL	NULL	NULL	p53	GP		bind					Mix.2 gene	GP	putative		p53-binding sites	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_development_130_17_3929_s_224	12874116	(A) p53 binds to the putative p53-binding sites from  Mix.2 gene in vitro.	bind
7191	1	3019	6	10	NULL	NULL	NULL	p53	GP		bind					Mix.2 gene	GP	putative		p53-binding site	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_development_130_17_3929_s_224	12874116	(A) p53 binds to the putative p53-binding sites from  Mix.2 gene in vitro.	bind
6689	1	3020	5	10	NULL	NULL	NULL	p55	GP		bind					 ARP53D	GP			E gene promoter 	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_9124_s_237	15456884	(A) p55 binds to the E gene promoter   ARP53D.	bind
7192	1	3020	6	10	NULL	NULL	NULL	p55	GP		bind					ARP53D	GP			E gene promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_9124_s_237	15456884	(A) p55 binds to the E gene promoter   ARP53D.	bind
6690	1	3021	5	10	NULL	NULL	NULL	p63	GP		bind					p73	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_8_3536_s_341	15060172	(A) p63 binds to p73 but not to p53.	bind
6691	2	3021	5	10	NULL	NULL	NULL	p63	GP		does not bind					p53	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_8_3536_s_341	15060172	(A) p63 binds to p73 but not to p53.	bind
7193	1	3021	6	10	NULL	NULL	NULL	p63	GP		bind					p73	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_8_3536_s_341	15060172	(A) p63 binds to p73 but not to p53.	bind
7195	2	3021	6	10	NULL	NULL	NULL	p63	GP		does not bind					p53	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_8_3536_s_341	15060172	(A) p63 binds to p73 but not to p53.	bind
6692	1	3022	5	10	NULL	NULL	NULL	p70 MGR	GP		bind					PCNA	GP	Drosophila		promoter	NULL		NULL	NULL	NULL	NULL	gw60_mechdev_114_1_37_s_150	12175488	(A) p70 MGR binds to the  Drosophila PCNA promoter.	bind
7197	1	3022	6	10	NULL	NULL	NULL	p70 MGR	GP		bind					PCNA	GP	drosophila		promoter	NULL		NULL	NULL	NULL	NULL	gw60_mechdev_114_1_37_s_150	12175488	(A) p70 MGR binds to the  Drosophila PCNA promoter.	bind
6693	1	3023	5	10	NULL	NULL	NULL	p97	GP		bind					c-Raf-1	GP	baculovirus			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_6_2235_s_200	11238956	(A) p97 binds c-Raf-1 from baculovirus.	bind
7198	1	3023	6	10	NULL	NULL	NULL	p97	GP		bind					c-Raf-1	GP	baculovirus			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_6_2235_s_200	11238956	(A) p97 binds c-Raf-1 from baculovirus.	bind
6694	1	3024	5	10	NULL	NULL	NULL	p97	GP		does not bind					MEK	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_6_2235_s_232	11238956	(A) p97 does not bind to MEK and is not activated by MEK.	bind
6695	2	3024	5	10	NULL	NULL	NULL	p97	GP		is not activated by					MEK	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_6_2235_s_232	11238956	(A) p97 does not bind to MEK and is not activated by MEK.	bind
7199	1	3024	6	10	NULL	NULL	NULL	p97	GP		does not bind					MEK	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_6_2235_s_232	11238956	(A) p97 does not bind to MEK and is not activated by MEK.	bind
7200	2	3024	6	10	NULL	NULL	NULL	p97	GP		is not activated by					MEK	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_6_2235_s_232	11238956	(A) p97 does not bind to MEK and is not activated by MEK.	bind
6696	1	3025	5	10	NULL	NULL	NULL	Par3L	GP		does not bind		detectably			PKC	GP				NULL		NULL	NULL	NULL	NULL	gw60_gene_294_1_99_s_195	12234671	(A) Par3L does not bind detectably to PKC .	bind
7201	1	3025	6	10	NULL	NULL	NULL	Par3L	GP		does not bind		detectably			PKC	GP				NULL		NULL	NULL	NULL	NULL	gw60_gene_294_1_99_s_195	12234671	(A) Par3L does not bind detectably to PKC .	bind
6697	1	3026	5	10	NULL	NULL	NULL	PARC	GP		bind					p53	GP				NULL	MEFs	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5579_s_219	15964813	(A) PARC binds p53 in MEFs.	bind
7202	1	3026	6	10	NULL	NULL	NULL	PARC	GP		bind					p53	GP				NULL	MEFs	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5579_s_219	15964813	(A) PARC binds p53 in MEFs.	bind
6698	1	3029	5	10	NULL	NULL	NULL	R1 peptide	AminoAcid		bind					AMA1	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_10_6981_s_161	16177378	(A) Phage  displaying the R1 peptide binding to immobilized AMA1 derived from a number of parasite  lines.	bind
67194	2	3029	5	10	NULL	NULL	NULL	AMA1	GP	immobilized	is derived from					parasite lines	Organism				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_10_6981_s_161	16177378	(A) Phage  displaying the R1 peptide binding to immobilized AMA1 derived from a number of parasite  lines.	bind
7203	1	3029	6	10	NULL	NULL	NULL	R1 peptide	AminoAcid		bind					AMA1	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_10_6981_s_161	16177378	(A) Phage  displaying the R1 peptide binding to immobilized AMA1 derived from a number of parasite  lines.	bind
7204	2	3029	6	10	NULL	NULL	NULL	AMA1	GP	immobilized	is derived from					parasite lines	Organism				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_10_6981_s_161	16177378	(A) Phage  displaying the R1 peptide binding to immobilized AMA1 derived from a number of parasite  lines.	bind
6699	1	3030	5	10	NULL	NULL	NULL	p47	GP	phosphorylated	bind					p97	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_161_6_1067_s_141	12810701	(A) Phosphorylated p47 binds to p97.	bind
7205	1	3030	6	10	NULL	NULL	NULL	p47	GP	phosphorylated	bind					p97	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_161_6_1067_s_141	12810701	(A) Phosphorylated p47 binds to p97.	bind
6700	1	3031	5	10	NULL	NULL	NULL	Ste11	GP		bind					Rad24	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_1_3_389_s_204	11702950	(A) Phosphorylation-dependent binding between Ste11 and Rad24.	bind
6701	2	3031	5	10	NULL	NULL	NULL	statement 1	Process		is dependent on					phosphorylation	Process				NULL		NULL	NULL	NULL	NULL	gw60_devcell_1_3_389_s_204	11702950	(A) Phosphorylation-dependent binding between Ste11 and Rad24.	bind
7206	1	3031	6	10	NULL	NULL	NULL	Ste11	GP		bind					Rad24	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_1_3_389_s_204	11702950	(A) Phosphorylation-dependent binding between Ste11 and Rad24.	bind
7207	2	3031	6	10	NULL	NULL	NULL	statement 1	Process		is dependent on					phosphorylation	Process				NULL		NULL	NULL	NULL	NULL	gw60_devcell_1_3_389_s_204	11702950	(A) Phosphorylation-dependent binding between Ste11 and Rad24.	bind
6702	1	3033	5	10	NULL	NULL	NULL	BAD	GP		bind					BCL-XL	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_1_41_s_211	10949026	(A) PKA and 14-3-3 cooperate to induce phosphorylation of BAD Ser-155 when BAD is bound to BCL-XL.	bind
6703	2	3033	5	10	NULL	NULL	NULL	PKA	GP		induce					BAD	GP	phosphorylation of	Ser-155		NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_1_41_s_211	10949026	(A) PKA and 14-3-3 cooperate to induce phosphorylation of BAD Ser-155 when BAD is bound to BCL-XL.	bind
6704	3	3033	5	10	NULL	NULL	NULL	14-3-3	GP		induce					BAD	GP	phosphorylation of	Ser-155		NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_1_41_s_211	10949026	(A) PKA and 14-3-3 cooperate to induce phosphorylation of BAD Ser-155 when BAD is bound to BCL-XL.	bind
6705	4	3033	5	10	NULL	NULL	NULL	statement 2	Process		occurs in cooperation with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_1_41_s_211	10949026	(A) PKA and 14-3-3 cooperate to induce phosphorylation of BAD Ser-155 when BAD is bound to BCL-XL.	bind
6706	5	3033	5	10	NULL	NULL	NULL	statement 4	Process		occurs following					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_1_41_s_211	10949026	(A) PKA and 14-3-3 cooperate to induce phosphorylation of BAD Ser-155 when BAD is bound to BCL-XL.	bind
7208	1	3033	6	10	NULL	NULL	NULL	PKA	GP		induce					BAD	GP	phosphorylation of	Ser-155		NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_1_41_s_211	10949026	(A) PKA and 14-3-3 cooperate to induce phosphorylation of BAD Ser-155 when BAD is bound to BCL-XL.	bind
7209	2	3033	6	10	NULL	NULL	NULL	14-3-3	GP		induce					BAD	GP	phosphorylation of	Ser-155		NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_1_41_s_211	10949026	(A) PKA and 14-3-3 cooperate to induce phosphorylation of BAD Ser-155 when BAD is bound to BCL-XL.	bind
7210	3	3033	6	10	NULL	NULL	NULL	statement 1	Process		occurs in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_1_41_s_211	10949026	(A) PKA and 14-3-3 cooperate to induce phosphorylation of BAD Ser-155 when BAD is bound to BCL-XL.	bind
7211	4	3033	6	10	NULL	NULL	NULL	BAD	GP		bind					BCL-XL	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_1_41_s_211	10949026	(A) PKA and 14-3-3 cooperate to induce phosphorylation of BAD Ser-155 when BAD is bound to BCL-XL.	bind
7212	5	3033	6	10	NULL	NULL	NULL	statement 4	Process		leads to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_1_41_s_211	10949026	(A) PKA and 14-3-3 cooperate to induce phosphorylation of BAD Ser-155 when BAD is bound to BCL-XL.	bind
7213	6	3033	6	10	NULL	NULL	NULL	statement 4	Process		leads to 					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_1_41_s_211	10949026	(A) PKA and 14-3-3 cooperate to induce phosphorylation of BAD Ser-155 when BAD is bound to BCL-XL.	bind
6707	1	3034	5	10	NULL	NULL	NULL	PKC	GP		bind					RACK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1487_2_163_s_243	11018469	(A) PKC  binding to RACK1 and peptide inhibited binding.	bind
8183	2	3034	5	10	NULL	NULL	NULL	peptide	AminoAcid		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1487_2_163_s_243	11018469	(A) PKC  binding to RACK1 and peptide inhibited binding.	bind
7214	1	3034	6	10	NULL	NULL	NULL	PKC	GP		bind					RACK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1487_2_163_s_243	11018469	(A) PKC  binding to RACK1 and peptide inhibited binding.	bind
7215	2	3034	6	10	NULL	NULL	NULL	peptide	AminoAcid		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1487_2_163_s_243	11018469	(A) PKC  binding to RACK1 and peptide inhibited binding.	bind
6708	3	3035	5	10	NULL	NULL	NULL	PKC	GP		bind		 	alpha C2 domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_56_s_161	16236797	(A) PKCalphaC2 domain and (B) cPLA2alphaC2 domain binding to phospholipid vesicles containing 3:1 PC:	bind
6709	2	3035	5	10	NULL	NULL	NULL	cPLA2	GP		bind			alpha C2 domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_56_s_161	16236797	(A) PKCalphaC2 domain and (B) cPLA2alphaC2 domain binding to phospholipid vesicles containing 3:1 PC:	bind
67195	1	3035	5	10	NULL	NULL	NULL	phospholipid vesicles \t	CellComponent		contains					PC	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_56_s_161	16236797	(A) PKCalphaC2 domain and (B) cPLA2alphaC2 domain binding to phospholipid vesicles containing 3:1 PC:	bind
7216	1	3035	6	10	NULL	NULL	NULL	phospholipid vesicles	CellComponent		contain					PC	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_56_s_161	16236797	(A) PKCalphaC2 domain and (B) cPLA2alphaC2 domain binding to phospholipid vesicles containing 3:1 PC:	bind
7217	2	3035	6	10	NULL	NULL	NULL	PKC	GP		bind			alpha C2 domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_56_s_161	16236797	(A) PKCalphaC2 domain and (B) cPLA2alphaC2 domain binding to phospholipid vesicles containing 3:1 PC:	bind
7218	3	3035	6	10	NULL	NULL	NULL	cPLA2	GP		bind			alpha C2 domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_56_s_161	16236797	(A) PKCalphaC2 domain and (B) cPLA2alphaC2 domain binding to phospholipid vesicles containing 3:1 PC:	bind
6710	1	3036	5	10	NULL	NULL	NULL	nuclear proteins	GP		bind									AP-1/TRE DNA-binding site	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3423_s_124	10207066	(A) PKD2 induces binding of nuclear proteins to the AP-1/TRE DNA-binding site.	bind
6711	2	3036	5	10	NULL	NULL	NULL	PKD2	GP		induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3423_s_124	10207066	(A) PKD2 induces binding of nuclear proteins to the AP-1/TRE DNA-binding site.	bind
7219	1	3036	6	10	NULL	NULL	NULL	nuclear proteins	GP		bind									AP-1/TRE DNA-binding site	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3423_s_124	10207066	(A) PKD2 induces binding of nuclear proteins to the AP-1/TRE DNA-binding site.	bind
7220	2	3036	6	10	NULL	NULL	NULL	PKD2	GP		induces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3423_s_124	10207066	(A) PKD2 induces binding of nuclear proteins to the AP-1/TRE DNA-binding site.	bind
6712	1	3038	5	10	NULL	NULL	NULL	anti-K18 peptide	GP		bind					SAg protein	GP				NULL	in solution	NULL	NULL	NULL	NULL	gw60_immunity_15_4_591_s_230	11672541	(A) Polyclonal anti-K18 peptide Abs bind the SAg protein in solution.	bind
53129	2	3038	5	10	NULL	NULL	NULL	anti-K18 peptide	GP		is a type of					polyclonal Ab	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_15_4_591_s_230	11672541	(A) Polyclonal anti-K18 peptide Abs bind the SAg protein in solution.	bind
7221	1	3038	6	10	NULL	NULL	NULL	anti-K18 peptide 	GP		bind					SAg protein	GP				NULL	in solution	NULL	NULL	NULL	NULL	gw60_immunity_15_4_591_s_230	11672541	(A) Polyclonal anti-K18 peptide Abs bind the SAg protein in solution.	bind
40685	2	3038	6	10	NULL	NULL	NULL	anti-K18 peptide	GP		is a type of					polyclonal Abs	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_15_4_591_s_230	11672541	(A) Polyclonal anti-K18 peptide Abs bind the SAg protein in solution.	bind
6713	1	3039	5	10	NULL	NULL	NULL	CF I 	GP		bind					pre-mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_11_6107_s_12	8626397	(A) polymerase (PAP) had no detectable effect on the binding of CF  I   to pre-mRNA.	bind
6714	2	3039	5	10	NULL	NULL	NULL	PAP	GP		does not effect					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_11_6107_s_12	8626397	(A) polymerase (PAP) had no detectable effect on the binding of CF  I   to pre-mRNA.	bind
53130	3	3039	5	10	NULL	NULL	NULL	PAP	GP		is a type of					polymerase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_11_6107_s_12	8626397	(A) polymerase (PAP) had no detectable effect on the binding of CF  I   to pre-mRNA.	bind
7222	1	3039	6	10	NULL	NULL	NULL	CF I	GP		bind					pre-mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_11_6107_s_12	8626397	(A) polymerase (PAP) had no detectable effect on the binding of CF  I   to pre-mRNA.	bind
7223	2	3039	6	10	NULL	NULL	NULL	PAP	GP		had no effect on					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_11_6107_s_12	8626397	(A) polymerase (PAP) had no detectable effect on the binding of CF  I   to pre-mRNA.	bind
53131	3	3039	6	10	NULL	NULL	NULL	PAP	GP		is a type of					polymerase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_11_6107_s_12	8626397	(A) polymerase (PAP) had no detectable effect on the binding of CF  I   to pre-mRNA.	bind
7146	1	3040	5	10	NULL	NULL	NULL	PAP	GP		is present					blastomeres	Cell	throughout			NULL		NULL	NULL	NULL	NULL	gw60_cell_103_3_435_s_107	11081630	(A) polymerase (PAP), and  the 100 kDa subunit of CPSF (the AAUAAA binding complex) were all detected  throughout the blastomeres, although there was a slight concentration of these proteins at  the centrosomes.	bind
7147	2	3040	5	10	NULL	NULL	NULL	CPSF	GP		is present			100 kDa subunit		blastomeres	Cell	throughout			NULL		NULL	NULL	NULL	NULL	gw60_cell_103_3_435_s_107	11081630	(A) polymerase (PAP), and  the 100 kDa subunit of CPSF (the AAUAAA binding complex) were all detected  throughout the blastomeres, although there was a slight concentration of these proteins at  the centrosomes.	bind
7148	3	3040	5	10	NULL	NULL	NULL	CPSF	GP		is			100 kDa subunit		AAUAAA binding complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_3_435_s_107	11081630	(A) polymerase (PAP), and  the 100 kDa subunit of CPSF (the AAUAAA binding complex) were all detected  throughout the blastomeres, although there was a slight concentration of these proteins at  the centrosomes.	bind
7149	4	3040	5	10	NULL	NULL	NULL	PAP	GP		is present in					centrosomes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_3_435_s_107	11081630	(A) polymerase (PAP), and  the 100 kDa subunit of CPSF (the AAUAAA binding complex) were all detected  throughout the blastomeres, although there was a slight concentration of these proteins at  the centrosomes.	bind
7150	5	3040	5	10	NULL	NULL	NULL	CPSF	GP		is present in			100 kDa subunit		centrosomes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_3_435_s_107	11081630	(A) polymerase (PAP), and  the 100 kDa subunit of CPSF (the AAUAAA binding complex) were all detected  throughout the blastomeres, although there was a slight concentration of these proteins at  the centrosomes.	bind
7224	1	3041	6	10	NULL	NULL	NULL	polymerase	GP		bind					pre-mRNA 	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_7_991_s_138	9651582	(A) polymerase or CstF binding to the pre-mRNA substrate (data not shown), the binding of CPSF to the L3 pre-mRNA precursor was prevented by the NS1 protein (  Figure 4).	bind
7225	2	3041	6	10	NULL	NULL	NULL	CstF	GP		bind					pre-mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_7_991_s_138	9651582	(A) polymerase or CstF binding to the pre-mRNA substrate (data not shown), the binding of CPSF to the L3 pre-mRNA precursor was prevented by the NS1 protein (  Figure 4).	bind
7226	3	3041	6	10	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_7_991_s_138	9651582	(A) polymerase or CstF binding to the pre-mRNA substrate (data not shown), the binding of CPSF to the L3 pre-mRNA precursor was prevented by the NS1 protein (  Figure 4).	bind
7227	4	3041	6	10	NULL	NULL	NULL	CPSF	GP		bind					L3 pre-mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_7_991_s_138	9651582	(A) polymerase or CstF binding to the pre-mRNA substrate (data not shown), the binding of CPSF to the L3 pre-mRNA precursor was prevented by the NS1 protein (  Figure 4).	bind
7228	5	3041	6	10	NULL	NULL	NULL	NS1 protein	GP		prevents					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_7_991_s_138	9651582	(A) polymerase or CstF binding to the pre-mRNA substrate (data not shown), the binding of CPSF to the L3 pre-mRNA precursor was prevented by the NS1 protein (  Figure 4).	bind
6748	1	3043	5	10	NULL	NULL	NULL	PP2A	GP	catalytically active 	bind					AR	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_4_1298_s_197	15684382	(A) PP2A bound to AR is catalytically  active.	bind
7229	1	3043	6	10	NULL	NULL	NULL	PP2A	GP	catalytically active	bind					AR	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_4_1298_s_197	15684382	(A) PP2A bound to AR is catalytically  active.	bind
6750	1	3044	5	10	NULL	NULL	NULL	Rac1	GP		bind					GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_18_6872_s_231	10958683	(A) Precipitation of FRL by the GTPgammaS- or GDP-bound form of Rac1.	bind
6751	2	3044	5	10	NULL	NULL	NULL	Rac1	GP		bind					GTPgammaS	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_18_6872_s_231	10958683	(A) Precipitation of FRL by the GTPgammaS- or GDP-bound form of Rac1.	bind
6752	3	3044	5	10	NULL	NULL	NULL	FRL	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_18_6872_s_231	10958683	(A) Precipitation of FRL by the GTPgammaS- or GDP-bound form of Rac1.	bind
6753	4	3044	5	10	NULL	NULL	NULL	FRL	GP		bind					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_18_6872_s_231	10958683	(A) Precipitation of FRL by the GTPgammaS- or GDP-bound form of Rac1.	bind
53135	5	3044	5	10	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_18_6872_s_231	10958683	(A) Precipitation of FRL by the GTPgammaS- or GDP-bound form of Rac1.	bind
7230	1	3044	6	10	NULL	NULL	NULL	Rac1	GP		bind					GTPgammaS	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_18_6872_s_231	10958683	(A) Precipitation of FRL by the GTPgammaS- or GDP-bound form of Rac1.	bind
7231	2	3044	6	10	NULL	NULL	NULL	 Rac1	GP		bind					GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_18_6872_s_231	10958683	(A) Precipitation of FRL by the GTPgammaS- or GDP-bound form of Rac1.	bind
7232	3	3044	6	10	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_18_6872_s_231	10958683	(A) Precipitation of FRL by the GTPgammaS- or GDP-bound form of Rac1.	bind
53132	4	3044	6	10	NULL	NULL	NULL	FRL	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_18_6872_s_231	10958683	(A) Precipitation of FRL by the GTPgammaS- or GDP-bound form of Rac1.	bind
53134	5	3044	6	10	NULL	NULL	NULL	FRL	GP		bind					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_18_6872_s_231	10958683	(A) Precipitation of FRL by the GTPgammaS- or GDP-bound form of Rac1.	bind
6754	1	3045	5	10	NULL	NULL	NULL	BCS1 precursor	GP		lacks								first 82 amino acid residues		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_7_2239_s_269	12640110	(A) Precursor lacking the first 82 amino acid residues of BCS1 can bind to OMV in a receptor-dependent manner.	bind
6755	2	3045	5	10	NULL	NULL	NULL	statement 1	Process		bind					OMV	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_7_2239_s_269	12640110	(A) Precursor lacking the first 82 amino acid residues of BCS1 can bind to OMV in a receptor-dependent manner.	bind
6756	3	3045	5	10	NULL	NULL	NULL	statement 2	Process		is dependent on					receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_7_2239_s_269	12640110	(A) Precursor lacking the first 82 amino acid residues of BCS1 can bind to OMV in a receptor-dependent manner.	bind
7233	1	3045	6	10	NULL	NULL	NULL	BCS1 precursor	GP		lacks								82 amino acid residues		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_7_2239_s_269	12640110	(A) Precursor lacking the first 82 amino acid residues of BCS1 can bind to OMV in a receptor-dependent manner.	bind
7234	2	3045	6	10	NULL	NULL	NULL	statement 1	Process		bind					OMV	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_7_2239_s_269	12640110	(A) Precursor lacking the first 82 amino acid residues of BCS1 can bind to OMV in a receptor-dependent manner.	bind
7235	3	3045	6	10	NULL	NULL	NULL	statement 2	Process		is dependent on					receptor 	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_7_2239_s_269	12640110	(A) Precursor lacking the first 82 amino acid residues of BCS1 can bind to OMV in a receptor-dependent manner.	bind
6757	1	3049	5	10	NULL	NULL	NULL	Arp2	GP		bind					nucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_2_315_s_245	15657399	(A) Proposed relative contributions of Arp2 and Arp3 nucleotide binding to actin  filament nucleation and a yet to be determined structural activity.	bind
6758	2	3049	5	10	NULL	NULL	NULL	Arp3	GP		bind					nucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_2_315_s_245	15657399	(A) Proposed relative contributions of Arp2 and Arp3 nucleotide binding to actin  filament nucleation and a yet to be determined structural activity.	bind
8184	3	3049	5	10	NULL	NULL	NULL	statement 1	Process		contribute to		may			actin filament	CellComponent	nucleation of			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_2_315_s_245	15657399	(A) Proposed relative contributions of Arp2 and Arp3 nucleotide binding to actin  filament nucleation and a yet to be determined structural activity.	bind
8185	4	3049	5	10	NULL	NULL	NULL	statement 2	Process		contribute to		may			actin filament	CellComponent	nucleation of			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_2_315_s_245	15657399	(A) Proposed relative contributions of Arp2 and Arp3 nucleotide binding to actin  filament nucleation and a yet to be determined structural activity.	bind
7236	1	3049	6	10	NULL	NULL	NULL	Arp2	GP		bind					nucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_2_315_s_245	15657399	(A) Proposed relative contributions of Arp2 and Arp3 nucleotide binding to actin  filament nucleation and a yet to be determined structural activity.	bind
7237	2	3049	6	10	NULL	NULL	NULL	Arp3	GP		bind					nucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_2_315_s_245	15657399	(A) Proposed relative contributions of Arp2 and Arp3 nucleotide binding to actin  filament nucleation and a yet to be determined structural activity.	bind
7238	3	3049	6	10	NULL	NULL	NULL	statement 1	Process		contribute in		may			actin filament	CellComponent	nucleation of 			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_2_315_s_245	15657399	(A) Proposed relative contributions of Arp2 and Arp3 nucleotide binding to actin  filament nucleation and a yet to be determined structural activity.	bind
7239	4	3049	6	10	NULL	NULL	NULL	statement 2	Process		contribute in		may			actin filament	CellComponent	nucleation of 			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_2_315_s_245	15657399	(A) Proposed relative contributions of Arp2 and Arp3 nucleotide binding to actin  filament nucleation and a yet to be determined structural activity.	bind
6759	1	3050	5	10	NULL	NULL	NULL	XARP	GP		associate with					Xdsh	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2228_s_219	10688669	(A) Protein complexes containing XARP in association with Xdsh did not significantly bind GSK3, whereas the pool of XARP that is not bound to Xdsh retained GSK3.	bind
6760	3	3050	5	10	NULL	NULL	NULL	statement 2	Process		does not bind		significantly			GSK3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2228_s_219	10688669	(A) Protein complexes containing XARP in association with Xdsh did not significantly bind GSK3, whereas the pool of XARP that is not bound to Xdsh retained GSK3.	bind
6761	4	3050	5	10	NULL	NULL	NULL	XARP	GP		bind					GSK3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2228_s_219	10688669	(A) Protein complexes containing XARP in association with Xdsh did not significantly bind GSK3, whereas the pool of XARP that is not bound to Xdsh retained GSK3.	bind
44734	2	3050	5	10	NULL	NULL	NULL	statement 1	Process		forms a 					complex					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2228_s_219	10688669	(A) Protein complexes containing XARP in association with Xdsh did not significantly bind GSK3, whereas the pool of XARP that is not bound to Xdsh retained GSK3.	bind
7247	1	3050	6	10	NULL	NULL	NULL	XARP	GP		associates					Xdsh	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2228_s_219	10688669	(A) Protein complexes containing XARP in association with Xdsh did not significantly bind GSK3, whereas the pool of XARP that is not bound to Xdsh retained GSK3.	bind
7248	2	3050	6	10	NULL	NULL	NULL	statement 1	Process		forms a 					complex					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2228_s_219	10688669	(A) Protein complexes containing XARP in association with Xdsh did not significantly bind GSK3, whereas the pool of XARP that is not bound to Xdsh retained GSK3.	bind
7249	3	3050	6	10	NULL	NULL	NULL	statement 2	Process		did not bind		significantly			GSK3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2228_s_219	10688669	(A) Protein complexes containing XARP in association with Xdsh did not significantly bind GSK3, whereas the pool of XARP that is not bound to Xdsh retained GSK3.	bind
7250	4	3050	6	10	NULL	NULL	NULL	XARP	GP		bind					GSK3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2228_s_219	10688669	(A) Protein complexes containing XARP in association with Xdsh did not significantly bind GSK3, whereas the pool of XARP that is not bound to Xdsh retained GSK3.	bind
6762	1	3051	5	10	NULL	NULL	NULL	rat brain subfraction protein	GP		bind					sAPP695T	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1571_3_225_s_186	12090937	(A) Proteins from rat brain subfractions that binds sAPP695T.	bind
7416	1	3051	6	10	NULL	NULL	NULL	rat brain subfraction protein	GP		bind					sAPP695T	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1571_3_225_s_186	12090937	(A) Proteins from rat brain subfractions that binds sAPP695T.	bind
6763	1	3052	5	10	NULL	NULL	NULL	nuclear extract protein	GP	HeLa cells	bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_21_9419_s_122	16227592	(a) Proteins in nuclear extracts  of HeLa cells that bound to GST (lane 3), GST-FGF-2 (lane 5), or GST-FGF-2 in the  presence of a 10-fold excess of hrFGF-2 (lane 6) were separated on a SDS-PAGE gel  and stained with Coomassie blue.	bind
6764	2	3052	5	10	NULL	NULL	NULL	nuclear extract protein	GP	HeLa cells	bind					GST-FGF-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_21_9419_s_122	16227592	(a) Proteins in nuclear extracts  of HeLa cells that bound to GST (lane 3), GST-FGF-2 (lane 5), or GST-FGF-2 in the  presence of a 10-fold excess of hrFGF-2 (lane 6) were separated on a SDS-PAGE gel  and stained with Coomassie blue.	bind
6765	3	3052	5	10	NULL	NULL	NULL	nuclear extract protein	GP	HeLa cells	bind					GST-FGF-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_21_9419_s_122	16227592	(a) Proteins in nuclear extracts  of HeLa cells that bound to GST (lane 3), GST-FGF-2 (lane 5), or GST-FGF-2 in the  presence of a 10-fold excess of hrFGF-2 (lane 6) were separated on a SDS-PAGE gel  and stained with Coomassie blue.	bind
44735	4	3052	5	10	NULL	NULL	NULL	statement 3	Process		occurs in presence of					hrFGF-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_21_9419_s_122	16227592	(a) Proteins in nuclear extracts  of HeLa cells that bound to GST (lane 3), GST-FGF-2 (lane 5), or GST-FGF-2 in the  presence of a 10-fold excess of hrFGF-2 (lane 6) were separated on a SDS-PAGE gel  and stained with Coomassie blue.	bind
7417	1	3052	6	10	NULL	NULL	NULL	nuclear extract protein	GP	HeLa cells	bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_21_9419_s_122	16227592	(a) Proteins in nuclear extracts  of HeLa cells that bound to GST (lane 3), GST-FGF-2 (lane 5), or GST-FGF-2 in the  presence of a 10-fold excess of hrFGF-2 (lane 6) were separated on a SDS-PAGE gel  and stained with Coomassie blue.	bind
7418	2	3052	6	10	NULL	NULL	NULL	nuclear extract protein	GP	HeLa cells	bind					GST-FGF-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_21_9419_s_122	16227592	(a) Proteins in nuclear extracts  of HeLa cells that bound to GST (lane 3), GST-FGF-2 (lane 5), or GST-FGF-2 in the  presence of a 10-fold excess of hrFGF-2 (lane 6) were separated on a SDS-PAGE gel  and stained with Coomassie blue.	bind
7419	3	3052	6	10	NULL	NULL	NULL	nuclear extract protein	GP	HeLa cells	bind					GST-FGF-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_21_9419_s_122	16227592	(a) Proteins in nuclear extracts  of HeLa cells that bound to GST (lane 3), GST-FGF-2 (lane 5), or GST-FGF-2 in the  presence of a 10-fold excess of hrFGF-2 (lane 6) were separated on a SDS-PAGE gel  and stained with Coomassie blue.	bind
44736	4	3052	6	10	NULL	NULL	NULL	statement 3	Process		occurs in presence of					hrFGF-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_21_9419_s_122	16227592	(a) Proteins in nuclear extracts  of HeLa cells that bound to GST (lane 3), GST-FGF-2 (lane 5), or GST-FGF-2 in the  presence of a 10-fold excess of hrFGF-2 (lane 6) were separated on a SDS-PAGE gel  and stained with Coomassie blue.	bind
6766	1	3053	5	10	NULL	NULL	NULL	Rac	GP		bind		selectively			PAK	GP		PBD-GST		NULL		NULL	NULL	NULL	NULL	gw60_neuron_33_5_741_s_55	11879651	(A) Pull-down assays showing that Rac is bound selectively by PBD-GST (PAK), RhoA is bound selectively by RBD-GST (Rhotekin), and Cdc42 is bound selectively by WBD-GST (WASP).	bind
6767	2	3053	5	10	NULL	NULL	NULL	RhoA	GP		bind		selectively			Rhotekin	GP		RBD-GST		NULL		NULL	NULL	NULL	NULL	gw60_neuron_33_5_741_s_55	11879651	(A) Pull-down assays showing that Rac is bound selectively by PBD-GST (PAK), RhoA is bound selectively by RBD-GST (Rhotekin), and Cdc42 is bound selectively by WBD-GST (WASP).	bind
6768	3	3053	5	10	NULL	NULL	NULL	Cdc42	GP		bind		selectively			WASP	GP		WBD-GST		NULL		NULL	NULL	NULL	NULL	gw60_neuron_33_5_741_s_55	11879651	(A) Pull-down assays showing that Rac is bound selectively by PBD-GST (PAK), RhoA is bound selectively by RBD-GST (Rhotekin), and Cdc42 is bound selectively by WBD-GST (WASP).	bind
7420	1	3053	6	10	NULL	NULL	NULL	Rac	GP		bind		selectively			PAK	GP		PBD-GST		NULL		NULL	NULL	NULL	NULL	gw60_neuron_33_5_741_s_55	11879651	(A) Pull-down assays showing that Rac is bound selectively by PBD-GST (PAK), RhoA is bound selectively by RBD-GST (Rhotekin), and Cdc42 is bound selectively by WBD-GST (WASP).	bind
7421	2	3053	6	10	NULL	NULL	NULL	RhoA	GP		bind		selectively			Rhotekin	GP		RBD-GST		NULL		NULL	NULL	NULL	NULL	gw60_neuron_33_5_741_s_55	11879651	(A) Pull-down assays showing that Rac is bound selectively by PBD-GST (PAK), RhoA is bound selectively by RBD-GST (Rhotekin), and Cdc42 is bound selectively by WBD-GST (WASP).	bind
7423	3	3053	6	10	NULL	NULL	NULL	Cdc42	GP		bind		selectively			WASP	GP		WBD-GST		NULL		NULL	NULL	NULL	NULL	gw60_neuron_33_5_741_s_55	11879651	(A) Pull-down assays showing that Rac is bound selectively by PBD-GST (PAK), RhoA is bound selectively by RBD-GST (Rhotekin), and Cdc42 is bound selectively by WBD-GST (WASP).	bind
6769	1	3056	5	10	NULL	NULL	NULL	(BV)Ase1p	GP	purified	bind		directly			MTs 	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_160_4_517_s_114	12591913	(A) Purified (BV)Ase1p binds MTs directly.	bind
7424	1	3056	6	10	NULL	NULL	NULL	Ase1p (BV)	GP	purified	bind		directly			MTs	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_160_4_517_s_114	12591913	(A) Purified (BV)Ase1p binds MTs directly.	bind
6770	1	3059	5	10	NULL	NULL	NULL	p53 protein	GP	Purified;; recombinant	bind							overlapping		HNF-3/p53 sites	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_2_1279_s_251	9891062	(A) Purified recombinant p53 protein binds to the overlapping HNF-3/p53 sites.	bind
7425	1	3059	6	10	NULL	NULL	NULL	p53 protein	GP	Purified;; recombinant	bind							overlapping		HNF-3/p53 sites	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_2_1279_s_251	9891062	(A) Purified recombinant p53 protein binds to the overlapping HNF-3/p53 sites.	bind
6771	1	3060	5	10	NULL	NULL	NULL	Sp1	GP		bind					bcl-2	GP			P1 promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1608_s_233	15713621	(A) Quantitative ChIP assays of the binding of Sp1, CREB,  and CBP to the  bcl-2 P1 promoter.	bind
6772	2	3060	5	10	NULL	NULL	NULL	CREB	GP		bind					 bcl-2	GP			P1 promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1608_s_233	15713621	(A) Quantitative ChIP assays of the binding of Sp1, CREB,  and CBP to the  bcl-2 P1 promoter.	bind
6773	3	3060	5	10	NULL	NULL	NULL	CBP	GP		bind					bcl-2	GP			P1 promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1608_s_233	15713621	(A) Quantitative ChIP assays of the binding of Sp1, CREB,  and CBP to the  bcl-2 P1 promoter.	bind
7426	1	3060	6	10	NULL	NULL	NULL	Sp1	GP		bind					bcl-2	GP			P1 promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1608_s_233	15713621	(A) Quantitative ChIP assays of the binding of Sp1, CREB,  and CBP to the  bcl-2 P1 promoter.	bind
7427	2	3060	6	10	NULL	NULL	NULL	CREB	GP		bind					bcl-2	GP			P1 promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1608_s_233	15713621	(A) Quantitative ChIP assays of the binding of Sp1, CREB,  and CBP to the  bcl-2 P1 promoter.	bind
7428	3	3060	6	10	NULL	NULL	NULL	CBP	GP		bind					bcl-2	GP			P1 promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1608_s_233	15713621	(A) Quantitative ChIP assays of the binding of Sp1, CREB,  and CBP to the  bcl-2 P1 promoter.	bind
6774	1	3061	5	10	NULL	NULL	NULL	Sec complex	GP		reconstituted into					proteoliposomes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cell_97_5_553_s_122	10367885	(A) Radiolabeled pp F was bound to Sec complex reconstituted into proteoliposomes.	bind
6775	2	3061	5	10	NULL	NULL	NULL	pp F	GP	radiolabelled	bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_97_5_553_s_122	10367885	(A) Radiolabeled pp F was bound to Sec complex reconstituted into proteoliposomes.	bind
7429	2	3061	6	10	NULL	NULL	NULL	pp F	GP	radiolabeled	bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_97_5_553_s_122	10367885	(A) Radiolabeled pp F was bound to Sec complex reconstituted into proteoliposomes.	bind
7430	1	3061	6	10	NULL	NULL	NULL	Sec complex	GP		reconstituted into					proteoliposomes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cell_97_5_553_s_122	10367885	(A) Radiolabeled pp F was bound to Sec complex reconstituted into proteoliposomes.	bind
6776	1	3062	5	10	NULL	NULL	NULL	SLC	GP		activate					Rap1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_161_2_417_s_40	12707305	(A) Rap1 activation by SLC.	bind
7431	1	3062	6	10	NULL	NULL	NULL	SLC	GP		activates					Rap1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_161_2_417_s_40	12707305	(A) Rap1 activation by SLC.	bind
10046	1	3063	5	10	NULL	NULL	NULL	Ras-GTP	GP		bind					Raf1	GP	GST tagged	RBD		NULL		NULL	NULL	NULL	NULL	gw70_febslett_579_2_455_s_214	15642358	(a) Ras activity in spreading NIH 3T3 fibroblasts was quantified  at different timepoints after plating on fibronectin as indicated, employing a Ras  activation assay based on Ras-GTP pulldowns using the GST-tagged Ras binding domain  (RBD) of Raf1.	bind
10047	2	3063	5	10	NULL	NULL	NULL	RBD	AminoAcid		is					Ras binding domain	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_febslett_579_2_455_s_214	15642358	(a) Ras activity in spreading NIH 3T3 fibroblasts was quantified  at different timepoints after plating on fibronectin as indicated, employing a Ras  activation assay based on Ras-GTP pulldowns using the GST-tagged Ras binding domain  (RBD) of Raf1.	bind
7749	1	3063	6	10	NULL	NULL	NULL	Ras-GTP	GP		bind					Raf1	GP	GST tagged	RBD		NULL		NULL	NULL	NULL	NULL	gw70_febslett_579_2_455_s_214	15642358	(a) Ras activity in spreading NIH 3T3 fibroblasts was quantified  at different timepoints after plating on fibronectin as indicated, employing a Ras  activation assay based on Ras-GTP pulldowns using the GST-tagged Ras binding domain  (RBD) of Raf1.	bind
7750	2	3063	6	10	NULL	NULL	NULL	RBD	AminoAcid		is					Ras binding domain	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_febslett_579_2_455_s_214	15642358	(a) Ras activity in spreading NIH 3T3 fibroblasts was quantified  at different timepoints after plating on fibronectin as indicated, employing a Ras  activation assay based on Ras-GTP pulldowns using the GST-tagged Ras binding domain  (RBD) of Raf1.	bind
6777	1	3065	5	10	NULL	NULL	NULL	RasG12V	GP		bind					MST1	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_4_253_s_139	11864565	(A) RasG12V binds MST1 through NORE1.	bind
6778	2	3065	5	10	NULL	NULL	NULL	statement 1	Process		occurs through					NORE1	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_4_253_s_139	11864565	(A) RasG12V binds MST1 through NORE1.	bind
7432	1	3065	6	10	NULL	NULL	NULL	RasG12V	GP		bind					MST1	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_4_253_s_139	11864565	(A) RasG12V binds MST1 through NORE1.	bind
8186	2	3065	6	10	NULL	NULL	NULL	statement 1	Process		occurs through					NORE1	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_4_253_s_139	11864565	(A) RasG12V binds MST1 through NORE1.	bind
6779	1	3067	5	10	NULL	NULL	NULL	3H-PREGS	Chemical		bind					GABA receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1619_3_301_s_757	12573490	(A) receptor:  3H-PREGS binding to GABA receptor.	bind
7433	1	3067	6	10	NULL	NULL	NULL	3H-PREGS	Chemical		bind					GABA receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1619_3_301_s_757	12573490	(A) receptor:  3H-PREGS binding to GABA receptor.	bind
6780	1	3068	5	10	NULL	NULL	NULL	IRP1	GP	Manduca;; recombinant	bind		specifically			ferritin	GP	M. sexta		IRE transcripts	NULL		NULL	NULL	NULL	NULL	gw60_insectbiochemmolbiol_32_1_85_s_185	11719072	(A) Recombinant  Manduca IRP1 binds specifically  M. sexta ferritin IRE transcripts.	bind
7434	1	3068	6	10	NULL	NULL	NULL	IRP1	GP	Manduca;; recombinant	bind		specifically			ferritin	GP	M.sexta		IRE transcripts	NULL		NULL	NULL	NULL	NULL	gw60_insectbiochemmolbiol_32_1_85_s_185	11719072	(A) Recombinant  Manduca IRP1 binds specifically  M. sexta ferritin IRE transcripts.	bind
6781	1	3070	5	10	NULL	NULL	NULL	IBP39	GP	recombinant	bind					ferredoxin	CellComponent	single		Inr element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_22_7872_s_274	11604521	(A) Recombinant IBP39 binds the ferredoxin single Inr element.	bind
7435	1	3070	6	10	NULL	NULL	NULL	IBP39	GP	recombinant	bind					ferredoxin	Chemical	single		Inr element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_22_7872_s_274	11604521	(A) Recombinant IBP39 binds the ferredoxin single Inr element.	bind
6782	1	3071	5	10	NULL	NULL	NULL	hrs	GP	recombinant	bind					actinin-4	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_5_2470_s_342	15772161	(A) Recombinant protein binding experiments suggest that there is an  ordered assembly for the complex: 1) hrs binds to actinin-4; 2) BERP binds to hrs/actinin-4;  and 3) myosin V binds to hrs/actinin-4/BERP.	bind
6783	2	3071	5	10	NULL	NULL	NULL	BERP	GP	recombinant	bind					hrs/actinin-4	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_5_2470_s_342	15772161	(A) Recombinant protein binding experiments suggest that there is an  ordered assembly for the complex: 1) hrs binds to actinin-4; 2) BERP binds to hrs/actinin-4;  and 3) myosin V binds to hrs/actinin-4/BERP.	bind
6784	3	3071	5	10	NULL	NULL	NULL	myosin V	GP	recombinant	bind					hrs/actinin-4/BERP	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_5_2470_s_342	15772161	(A) Recombinant protein binding experiments suggest that there is an  ordered assembly for the complex: 1) hrs binds to actinin-4; 2) BERP binds to hrs/actinin-4;  and 3) myosin V binds to hrs/actinin-4/BERP.	bind
7486	1	3071	6	10	NULL	NULL	NULL	hrs	GP	recombinant	bind					actinin-4	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_5_2470_s_342	15772161	(A) Recombinant protein binding experiments suggest that there is an  ordered assembly for the complex: 1) hrs binds to actinin-4; 2) BERP binds to hrs/actinin-4;  and 3) myosin V binds to hrs/actinin-4/BERP.	bind
7487	2	3071	6	10	NULL	NULL	NULL	BERP	GP	recombinant	bind					hrs/actinin-4	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_5_2470_s_342	15772161	(A) Recombinant protein binding experiments suggest that there is an  ordered assembly for the complex: 1) hrs binds to actinin-4; 2) BERP binds to hrs/actinin-4;  and 3) myosin V binds to hrs/actinin-4/BERP.	bind
7488	3	3071	6	10	NULL	NULL	NULL	myosin V	GP	recombinant	bind					hrs/actinin-4/BERP	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_5_2470_s_342	15772161	(A) Recombinant protein binding experiments suggest that there is an  ordered assembly for the complex: 1) hrs binds to actinin-4; 2) BERP binds to hrs/actinin-4;  and 3) myosin V binds to hrs/actinin-4/BERP.	bind
6785	1	3072	5	10	NULL	NULL	NULL	SWI/SNF	GP	recruitment of	results in					protein A	GP	stabilized binding of			NULL		NULL	NULL	NULL	NULL	gw60_cell_109_3_267_s_122	12015975	(A) recruits a chromatin-remodeling complex (SWI/SNF), which results in stabilized binding of protein A through an ATP-dependent perturbation of nucleosomal structure.	bind
6786	2	3072	5	10	NULL	NULL	NULL	SWI/SNF	GP		is a type of					chromatin-remodeling complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_109_3_267_s_122	12015975	(A) recruits a chromatin-remodeling complex (SWI/SNF), which results in stabilized binding of protein A through an ATP-dependent perturbation of nucleosomal structure.	bind
6787	3	3072	5	10	NULL	NULL	NULL	nucleosomal structure	CellComponent	perturbation of	is dependent on					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_109_3_267_s_122	12015975	(A) recruits a chromatin-remodeling complex (SWI/SNF), which results in stabilized binding of protein A through an ATP-dependent perturbation of nucleosomal structure.	bind
44740	4	3072	5	10	NULL	NULL	NULL	statement 1	Process		occurs through					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_109_3_267_s_122	12015975	(A) recruits a chromatin-remodeling complex (SWI/SNF), which results in stabilized binding of protein A through an ATP-dependent perturbation of nucleosomal structure.	bind
7436	1	3072	6	10	NULL	NULL	NULL	SWI/SNF	GP		is a type of					chromatin-remodeling complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_109_3_267_s_122	12015975	(A) recruits a chromatin-remodeling complex (SWI/SNF), which results in stabilized binding of protein A through an ATP-dependent perturbation of nucleosomal structure.	bind
7437	2	3072	6	10	NULL	NULL	NULL	SWI/SNF	GP	recruitment of	results in					Protein A	GP	stabilized binding of			NULL		NULL	NULL	NULL	NULL	gw60_cell_109_3_267_s_122	12015975	(A) recruits a chromatin-remodeling complex (SWI/SNF), which results in stabilized binding of protein A through an ATP-dependent perturbation of nucleosomal structure.	bind
7438	3	3072	6	10	NULL	NULL	NULL	nucleosomal structure	CellComponent	perturbation of	is dependent on					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_109_3_267_s_122	12015975	(A) recruits a chromatin-remodeling complex (SWI/SNF), which results in stabilized binding of protein A through an ATP-dependent perturbation of nucleosomal structure.	bind
7439	4	3072	6	10	NULL	NULL	NULL	statement 2	Process		occurs through					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_109_3_267_s_122	12015975	(A) recruits a chromatin-remodeling complex (SWI/SNF), which results in stabilized binding of protein A through an ATP-dependent perturbation of nucleosomal structure.	bind
6788	1	3073	5	10	NULL	NULL	NULL	rhodanese	GP		bind					EL229C	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_71	11672529	(A) Refolding  of 0.5 muM rhodanese bound to either  0.5 muM EL229C ( ) or EL229C-B ( ) in the  presence of 1 muM GroES and 5  mM ATP.	bind
6789	2	3073	5	10	NULL	NULL	NULL	statement 1	Process		in the presence of					GroES	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_71	11672529	(A) Refolding  of 0.5 muM rhodanese bound to either  0.5 muM EL229C ( ) or EL229C-B ( ) in the  presence of 1 muM GroES and 5  mM ATP.	bind
6790	3	3073	5	10	NULL	NULL	NULL	statement 1	Process		in the presence of					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_71	11672529	(A) Refolding  of 0.5 muM rhodanese bound to either  0.5 muM EL229C ( ) or EL229C-B ( ) in the  presence of 1 muM GroES and 5  mM ATP.	bind
6791	4	3073	5	10	NULL	NULL	NULL	rhodanese	GP		bind					EL229C-B	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_71	11672529	(A) Refolding  of 0.5 muM rhodanese bound to either  0.5 muM EL229C ( ) or EL229C-B ( ) in the  presence of 1 muM GroES and 5  mM ATP.	bind
6792	5	3073	5	10	NULL	NULL	NULL	statement 4	Process		in the presence of					GroES	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_71	11672529	(A) Refolding  of 0.5 muM rhodanese bound to either  0.5 muM EL229C ( ) or EL229C-B ( ) in the  presence of 1 muM GroES and 5  mM ATP.	bind
6793	6	3073	5	10	NULL	NULL	NULL	statement 4	Process		in the presence of					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_71	11672529	(A) Refolding  of 0.5 muM rhodanese bound to either  0.5 muM EL229C ( ) or EL229C-B ( ) in the  presence of 1 muM GroES and 5  mM ATP.	bind
6794	7	3073	5	10	NULL	NULL	NULL	statement 2	Process		undergoes					refolding	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_71	11672529	(A) Refolding  of 0.5 muM rhodanese bound to either  0.5 muM EL229C ( ) or EL229C-B ( ) in the  presence of 1 muM GroES and 5  mM ATP.	bind
6795	8	3073	5	10	NULL	NULL	NULL	statement 3	Process		undergoes					refolding	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_71	11672529	(A) Refolding  of 0.5 muM rhodanese bound to either  0.5 muM EL229C ( ) or EL229C-B ( ) in the  presence of 1 muM GroES and 5  mM ATP.	bind
6796	9	3073	5	10	NULL	NULL	NULL	statement 6	Process		undergoes					refolding	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_71	11672529	(A) Refolding  of 0.5 muM rhodanese bound to either  0.5 muM EL229C ( ) or EL229C-B ( ) in the  presence of 1 muM GroES and 5  mM ATP.	bind
6797	10	3073	5	10	NULL	NULL	NULL	statement 7	Process		undergoes					refolding	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_71	11672529	(A) Refolding  of 0.5 muM rhodanese bound to either  0.5 muM EL229C ( ) or EL229C-B ( ) in the  presence of 1 muM GroES and 5  mM ATP.	bind
7712	1	3073	6	10	NULL	NULL	NULL	rhodanese	GP		bind					EL229C	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_71	11672529	(A) Refolding  of 0.5 muM rhodanese bound to either  0.5 muM EL229C ( ) or EL229C-B ( ) in the  presence of 1 muM GroES and 5  mM ATP.	bind
7713	2	3073	6	10	NULL	NULL	NULL	rhodanese	GP		bind					EL229C-B	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_71	11672529	(A) Refolding  of 0.5 muM rhodanese bound to either  0.5 muM EL229C ( ) or EL229C-B ( ) in the  presence of 1 muM GroES and 5  mM ATP.	bind
7714	3	3073	6	10	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_71	11672529	(A) Refolding  of 0.5 muM rhodanese bound to either  0.5 muM EL229C ( ) or EL229C-B ( ) in the  presence of 1 muM GroES and 5  mM ATP.	bind
7715	4	3073	6	10	NULL	NULL	NULL	statement 1	Process		occurs in presence of					GroES	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_71	11672529	(A) Refolding  of 0.5 muM rhodanese bound to either  0.5 muM EL229C ( ) or EL229C-B ( ) in the  presence of 1 muM GroES and 5  mM ATP.	bind
7716	5	3073	6	10	NULL	NULL	NULL	statement 2	Process		occurs in presence of					GroES	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_71	11672529	(A) Refolding  of 0.5 muM rhodanese bound to either  0.5 muM EL229C ( ) or EL229C-B ( ) in the  presence of 1 muM GroES and 5  mM ATP.	bind
7717	6	3073	6	10	NULL	NULL	NULL	statement 1	Process		occurs in presence of					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_71	11672529	(A) Refolding  of 0.5 muM rhodanese bound to either  0.5 muM EL229C ( ) or EL229C-B ( ) in the  presence of 1 muM GroES and 5  mM ATP.	bind
7718	7	3073	6	10	NULL	NULL	NULL	statement 2	Process		occurs in presence of					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_71	11672529	(A) Refolding  of 0.5 muM rhodanese bound to either  0.5 muM EL229C ( ) or EL229C-B ( ) in the  presence of 1 muM GroES and 5  mM ATP.	bind
9692	8	3073	6	10	NULL	NULL	NULL	rhodanese	GP	refolding of	occurs during					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_71	11672529	(A) Refolding  of 0.5 muM rhodanese bound to either  0.5 muM EL229C ( ) or EL229C-B ( ) in the  presence of 1 muM GroES and 5  mM ATP.	bind
9693	9	3073	6	10	NULL	NULL	NULL	rhodanese	GP	refolding of	occurs during					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_71	11672529	(A) Refolding  of 0.5 muM rhodanese bound to either  0.5 muM EL229C ( ) or EL229C-B ( ) in the  presence of 1 muM GroES and 5  mM ATP.	bind
6829	1	3075	5	10	NULL	NULL	NULL	bilirubin	Chemical		bind					HSA	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1750_1_93_s_151	15890566	(A) Relative fluorescence of bilirubin bound to HSA in the presence of 0.0  M ( ), 1.2 M ( ), 2.2 M () and 2.4 M ( ) and 6.0 M ( ) GnHCl.	bind
6830	2	3075	5	10	NULL	NULL	NULL	statement 1	Process		in the presence of					GnHCl	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1750_1_93_s_151	15890566	(A) Relative fluorescence of bilirubin bound to HSA in the presence of 0.0  M ( ), 1.2 M ( ), 2.2 M () and 2.4 M ( ) and 6.0 M ( ) GnHCl.	bind
7489	1	3075	6	10	NULL	NULL	NULL	bilirubin	Chemical		bind					HSA	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1750_1_93_s_151	15890566	(A) Relative fluorescence of bilirubin bound to HSA in the presence of 0.0  M ( ), 1.2 M ( ), 2.2 M () and 2.4 M ( ) and 6.0 M ( ) GnHCl.	bind
7492	2	3075	6	10	NULL	NULL	NULL	statement 1	Process		occurs in presence of					GnHCl	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1750_1_93_s_151	15890566	(A) Relative fluorescence of bilirubin bound to HSA in the presence of 0.0  M ( ), 1.2 M ( ), 2.2 M () and 2.4 M ( ) and 6.0 M ( ) GnHCl.	bind
6831	1	3077	5	10	NULL	NULL	NULL	fraction S	NucleicAcid		bind					anti-Z-DNA antibody	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_14_5382_s_271	16809774	(A) Relaxed minicircles; (B) fraction S minicircles; (C)  fraction S bound to anti-Z-DNA antibody; (D) fraction S bound to SSB.	bind
6832	2	3077	5	10	NULL	NULL	NULL	fraction S	NucleicAcid		bind					SSB	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_14_5382_s_271	16809774	(A) Relaxed minicircles; (B) fraction S minicircles; (C)  fraction S bound to anti-Z-DNA antibody; (D) fraction S bound to SSB.	bind
7493	1	3077	6	10	NULL	NULL	NULL	fraction S	NucleicAcid		bind					anti-Z-DNA antibody	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_14_5382_s_271	16809774	(A) Relaxed minicircles; (B) fraction S minicircles; (C)  fraction S bound to anti-Z-DNA antibody; (D) fraction S bound to SSB.	bind
7494	2	3077	6	10	NULL	NULL	NULL	fraction S	NucleicAcid		bind					SSB	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_14_5382_s_271	16809774	(A) Relaxed minicircles; (B) fraction S minicircles; (C)  fraction S bound to anti-Z-DNA antibody; (D) fraction S bound to SSB.	bind
6858	1	3078	5	10	NULL	NULL	NULL	phage A1-10	Organism		bind					OppA-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_1_51_s_217	14679224	(A) Representative  dose-response graph of peptide inhibition of binding of phage A1-10 to OppA-1.	bind
7496	1	3078	6	10	NULL	NULL	NULL	phage A1-10	Organism		bind					OppA-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_1_51_s_217	14679224	(A) Representative  dose-response graph of peptide inhibition of binding of phage A1-10 to OppA-1.	bind
6859	1	3079	5	10	NULL	NULL	NULL	Hal3p	GP		bind					Ppz1deltaN-GST	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8683_s_203	16166647	(A) Representative  Western blot showing the amount of Hal3p (top) or Ypi1p (bottom) bound by the Ppz1deltaN-GST affinity resin at the pH indicated and the amount of Hal3p or Ypi1p in the starting  extracts (input).	bind
6860	2	3079	5	10	NULL	NULL	NULL	Ypi1p	GP		bind					Ppz1deltaN-GST	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8683_s_203	16166647	(A) Representative  Western blot showing the amount of Hal3p (top) or Ypi1p (bottom) bound by the Ppz1deltaN-GST affinity resin at the pH indicated and the amount of Hal3p or Ypi1p in the starting  extracts (input).	bind
53136	3	3079	5	10	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8683_s_203	16166647	(A) Representative  Western blot showing the amount of Hal3p (top) or Ypi1p (bottom) bound by the Ppz1deltaN-GST affinity resin at the pH indicated and the amount of Hal3p or Ypi1p in the starting  extracts (input).	bind
7498	1	3079	6	10	NULL	NULL	NULL	Hal3p	GP		bind					Ppz1deltaN-GST	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8683_s_203	16166647	(A) Representative  Western blot showing the amount of Hal3p (top) or Ypi1p (bottom) bound by the Ppz1deltaN-GST affinity resin at the pH indicated and the amount of Hal3p or Ypi1p in the starting  extracts (input).	bind
7499	2	3079	6	10	NULL	NULL	NULL	Ypi1p	GP		bind					Ppz1deltaN-GST	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8683_s_203	16166647	(A) Representative  Western blot showing the amount of Hal3p (top) or Ypi1p (bottom) bound by the Ppz1deltaN-GST affinity resin at the pH indicated and the amount of Hal3p or Ypi1p in the starting  extracts (input).	bind
7500	3	3079	6	10	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8683_s_203	16166647	(A) Representative  Western blot showing the amount of Hal3p (top) or Ypi1p (bottom) bound by the Ppz1deltaN-GST affinity resin at the pH indicated and the amount of Hal3p or Ypi1p in the starting  extracts (input).	bind
6908	1	3080	5	10	NULL	NULL	NULL	TBPS	Chemical		bind					C57BL/6 brain sections	OrganismPart	mouse 			NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_48_4_469_s_141	15755475	(A) Representative autoradiographic images of [35]TBPS binding to C57BL/6 and  2I77 mouse brain sections in the presence and absence  of 0.5  M GABA and 30  M DMCM. Gr, granule cell layer; Mol, molecular layer; (B)  quantitative results of the regions.	bind
6913	2	3080	5	10	NULL	NULL	NULL	TBPS	Chemical		bind					2I77 brain sections	OrganismPart	mouse 			NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_48_4_469_s_141	15755475	(A) Representative autoradiographic images of [35]TBPS binding to C57BL/6 and  2I77 mouse brain sections in the presence and absence  of 0.5  M GABA and 30  M DMCM. Gr, granule cell layer; Mol, molecular layer; (B)  quantitative results of the regions.	bind
7501	1	3080	6	10	NULL	NULL	NULL	TBPS	Chemical		bind					C57BL/6 brain sections	OrganismPart	mouse 			NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_48_4_469_s_141	15755475	(A) Representative autoradiographic images of [35]TBPS binding to C57BL/6 and  2I77 mouse brain sections in the presence and absence  of 0.5  M GABA and 30  M DMCM. Gr, granule cell layer; Mol, molecular layer; (B)  quantitative results of the regions.	bind
7502	2	3080	6	10	NULL	NULL	NULL	TBPS	Chemical		bind					2I77 brain sections	OrganismPart	mouse			NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_48_4_469_s_141	15755475	(A) Representative autoradiographic images of [35]TBPS binding to C57BL/6 and  2I77 mouse brain sections in the presence and absence  of 0.5  M GABA and 30  M DMCM. Gr, granule cell layer; Mol, molecular layer; (B)  quantitative results of the regions.	bind
6930	1	3082	5	10	NULL	NULL	NULL	Mot1p	GP		bind					HXT genes	GP				NULL	wild-type cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_4863_s_167	15923605	(A) Representative PCR and PhosphorImager  quantification of Mot1p binding to  HXT genes in wild-type (Wt),  gcn5delta,  spt3delta, and  spt8delta cells.	bind
6931	2	3082	5	10	NULL	NULL	NULL	Mot1p	GP		bind					HXT genes	GP				NULL	gcn5delta cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_4863_s_167	15923605	(A) Representative PCR and PhosphorImager  quantification of Mot1p binding to  HXT genes in wild-type (Wt),  gcn5delta,  spt3delta, and  spt8delta cells.	bind
6932	3	3082	5	10	NULL	NULL	NULL	Mot1p	GP		bind					HXT genes	GP				NULL	spt3delta cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_4863_s_167	15923605	(A) Representative PCR and PhosphorImager  quantification of Mot1p binding to  HXT genes in wild-type (Wt),  gcn5delta,  spt3delta, and  spt8delta cells.	bind
6933	4	3082	5	10	NULL	NULL	NULL	Mot1p	GP		bind					HXT genes	GP				NULL	spt8delta cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_4863_s_167	15923605	(A) Representative PCR and PhosphorImager  quantification of Mot1p binding to  HXT genes in wild-type (Wt),  gcn5delta,  spt3delta, and  spt8delta cells.	bind
7503	1	3082	6	10	NULL	NULL	NULL	Mot1p	GP		bind					HXT genes	GP				NULL	wild type cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_4863_s_167	15923605	(A) Representative PCR and PhosphorImager  quantification of Mot1p binding to  HXT genes in wild-type (Wt),  gcn5delta,  spt3delta, and  spt8delta cells.	bind
7504	2	3082	6	10	NULL	NULL	NULL	Mot1p	GP		bind					HXT genes	GP				NULL	gcn5delta cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_4863_s_167	15923605	(A) Representative PCR and PhosphorImager  quantification of Mot1p binding to  HXT genes in wild-type (Wt),  gcn5delta,  spt3delta, and  spt8delta cells.	bind
7505	3	3082	6	10	NULL	NULL	NULL	Mot1p	GP		bind					HXT genes	GP				NULL	spt3delta cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_4863_s_167	15923605	(A) Representative PCR and PhosphorImager  quantification of Mot1p binding to  HXT genes in wild-type (Wt),  gcn5delta,  spt3delta, and  spt8delta cells.	bind
7506	4	3082	6	10	NULL	NULL	NULL	Mot1p	GP		bind					HXT genes	GP				NULL	spt8delta cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_4863_s_167	15923605	(A) Representative PCR and PhosphorImager  quantification of Mot1p binding to  HXT genes in wild-type (Wt),  gcn5delta,  spt3delta, and  spt8delta cells.	bind
6934	1	3085	5	10	NULL	NULL	NULL	apoB-100	GP		bind					apo[a]	GP				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_46_4_769_s_159	15654123	(A) resulted in high-levels of Lp[a, with most of  the apoB-100 bound to apo[a (C).	bind
7507	1	3085	6	10	NULL	NULL	NULL	apoB-100	GP		bind					apo[a]	GP				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_46_4_769_s_159	15654123	(A) resulted in high-levels of Lp[a, with most of  the apoB-100 bound to apo[a (C).	bind
6936	1	3086	5	10	NULL	NULL	NULL	CodY	GP		bind					PD-3	NucleicAcid			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_10_3118_s_196	12730172	(A) Results of  CodY binding to PD-3, the sigmaD-dependent promoter.	bind
44741	2	3086	5	10	NULL	NULL	NULL	PD-3	NucleicAcid		is dependent on					sigmaD	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_10_3118_s_196	12730172	(A) Results of  CodY binding to PD-3, the sigmaD-dependent promoter.	bind
7508	1	3086	6	10	NULL	NULL	NULL	PD-3	NucleicAcid		is dependent on					sigmaD	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_10_3118_s_196	12730172	(A) Results of  CodY binding to PD-3, the sigmaD-dependent promoter.	bind
7509	2	3086	6	10	NULL	NULL	NULL	CodY	GP		bind					PD-3	NucleicAcid			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_10_3118_s_196	12730172	(A) Results of  CodY binding to PD-3, the sigmaD-dependent promoter.	bind
6938	1	3089	5	10	NULL	NULL	NULL	rIB2	GP		bind					MKK3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4073_s_192	12024021	(A) rIB2 binds to MKK3.	bind
7512	1	3089	6	10	NULL	NULL	NULL	rIB2	GP		bind					MKK3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4073_s_192	12024021	(A) rIB2 binds to MKK3.	bind
6941	1	3090	5	10	NULL	NULL	NULL	RXR	GP		bind			LBD		SRC-1	GP		LxxLL motif		NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_3_545_s_122	10882139	(a) Ribbon drawings of the RXR  LBD bound to the SRC-1 LxxLL motif (magenta) and 9cRA.	bind
6942	2	3090	5	10	NULL	NULL	NULL	RXR	GP		bind			LBD		9cRA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_3_545_s_122	10882139	(a) Ribbon drawings of the RXR  LBD bound to the SRC-1 LxxLL motif (magenta) and 9cRA.	bind
7513	1	3090	6	10	NULL	NULL	NULL	RXR	GP		bind			LBD		SRC-1	GP		LxxLL motif		NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_3_545_s_122	10882139	(a) Ribbon drawings of the RXR  LBD bound to the SRC-1 LxxLL motif (magenta) and 9cRA.	bind
7514	2	3090	6	10	NULL	NULL	NULL	RXR	GP		bind			LBD		9cRA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_3_545_s_122	10882139	(a) Ribbon drawings of the RXR  LBD bound to the SRC-1 LxxLL motif (magenta) and 9cRA.	bind
6943	1	3092	5	10	NULL	NULL	NULL	HP0525	GP		bind					ADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_7_1919_s_84	15028675	(A) Ribbon presentation of  HP0525 bound to ADP.	bind
7515	1	3092	6	10	NULL	NULL	NULL	HP0525	GP		bind					ADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_7_1919_s_84	15028675	(A) Ribbon presentation of  HP0525 bound to ADP.	bind
6946	1	3093	5	10	NULL	NULL	NULL	ARF1t	GP	nucleotide-free;; human	bind					Gea2	GP	yeast	Sec7 domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_95_2_237_s_151	9790530	(A) Ribbon representation of nucleotide-free human ARF1t (blue) bound  to the Sec7 domain of yeast Gea2 (pink).	bind
7516	1	3093	6	10	NULL	NULL	NULL	ARF1t	GP	nucleotide-free;; human	bind					Gea2	GP	yeast	Sec7 domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_95_2_237_s_151	9790530	(A) Ribbon representation of nucleotide-free human ARF1t (blue) bound  to the Sec7 domain of yeast Gea2 (pink).	bind
6947	1	3095	5	10	NULL	NULL	NULL	Rifampin	Chemical		bind					TL	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1688_2_102_s_101	14990340	(A) Rifampin binding to TL.	bind
7517	1	3095	6	10	NULL	NULL	NULL	Rifampin	Chemical		bind					TL	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1688_2_102_s_101	14990340	(A) Rifampin binding to TL.	bind
6948	1	3096	5	10	NULL	NULL	NULL	Rig protein	GP		bind					DHR3	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_development_131_1_25_s_202	14645129	(A) Rig protein binds to DHR3, EcR, betaFTZ-F1, USP and SVP in vitro.	bind
6949	2	3096	5	10	NULL	NULL	NULL	Rig protein	GP		bind					EcR	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_development_131_1_25_s_202	14645129	(A) Rig protein binds to DHR3, EcR, betaFTZ-F1, USP and SVP in vitro.	bind
6952	3	3096	5	10	NULL	NULL	NULL	Rig protein	GP		bind					betaFTZ-F1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_development_131_1_25_s_202	14645129	(A) Rig protein binds to DHR3, EcR, betaFTZ-F1, USP and SVP in vitro.	bind
6953	4	3096	5	10	NULL	NULL	NULL	Rig protein	GP		bind					USP	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_development_131_1_25_s_202	14645129	(A) Rig protein binds to DHR3, EcR, betaFTZ-F1, USP and SVP in vitro.	bind
6955	5	3096	5	10	NULL	NULL	NULL	Rig protein	GP		bind					SVP	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_development_131_1_25_s_202	14645129	(A) Rig protein binds to DHR3, EcR, betaFTZ-F1, USP and SVP in vitro.	bind
7518	1	3096	6	10	NULL	NULL	NULL	Rig protein	GP		bind					DHR3	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_development_131_1_25_s_202	14645129	(A) Rig protein binds to DHR3, EcR, betaFTZ-F1, USP and SVP in vitro.	bind
7519	2	3096	6	10	NULL	NULL	NULL	Rig protein	GP		bind					EcR	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_development_131_1_25_s_202	14645129	(A) Rig protein binds to DHR3, EcR, betaFTZ-F1, USP and SVP in vitro.	bind
7520	3	3096	6	10	NULL	NULL	NULL	Rig protein	GP		bind					betaFTZ-F1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_development_131_1_25_s_202	14645129	(A) Rig protein binds to DHR3, EcR, betaFTZ-F1, USP and SVP in vitro.	bind
7521	4	3096	6	10	NULL	NULL	NULL	Rig protein	GP		bind					USP	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_development_131_1_25_s_202	14645129	(A) Rig protein binds to DHR3, EcR, betaFTZ-F1, USP and SVP in vitro.	bind
7522	5	3096	6	10	NULL	NULL	NULL	Rig protein	GP		bind					SVP	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_development_131_1_25_s_202	14645129	(A) Rig protein binds to DHR3, EcR, betaFTZ-F1, USP and SVP in vitro.	bind
6956	1	3097	5	10	NULL	NULL	NULL	RIP2	GP		bind					caspase-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_99_s_173	11051551	(A) RIP2 binds  caspase-1 in an LPS-dependent manner (upper panel, lane 3 versus lane 1).	bind
6957	2	3097	5	10	NULL	NULL	NULL	statement 1	Process		is dependent on					LPS	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_99_s_173	11051551	(A) RIP2 binds  caspase-1 in an LPS-dependent manner (upper panel, lane 3 versus lane 1).	bind
7523	1	3097	6	10	NULL	NULL	NULL	RIP2	GP		bind					caspase-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_99_s_173	11051551	(A) RIP2 binds  caspase-1 in an LPS-dependent manner (upper panel, lane 3 versus lane 1).	bind
7524	2	3097	6	10	NULL	NULL	NULL	statement 1	Process		is dependent on					LPS	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_99_s_173	11051551	(A) RIP2 binds  caspase-1 in an LPS-dependent manner (upper panel, lane 3 versus lane 1).	bind
6958	1	3098	5	10	NULL	NULL	NULL	RIP2	GP		bind					caspase-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_99_s_89	11051551	(A) RIP2 binds caspase-1 (left and right upper panels).	bind
7525	1	3098	6	10	NULL	NULL	NULL	RIP2	GP		bind					caspase-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_99_s_89	11051551	(A) RIP2 binds caspase-1 (left and right upper panels).	bind
79247	1	3100	11	NULL	NULL	0	NULL	RNA	NucleicAcidSubstance		is a part of 					RNase P assay	ResearchActivity				NULL		0	NULL	NULL	NULL	gw60_febslett_511_1_107_s_112	11821058	(A) RNA in the RNase P assay, we sought to provide a competitor RNA that could bind NeoR or R3G through non-specific, electrostatic interactions and thus reduce their availability for similar interactions with the ptRNA substrate.	bind
7312	1	3102	5	11	NULL	0	NULL	RNA polymerase II 	GP		paused at					arrest site	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_12_4046_s_279	12773550	(A) RNA polymerase II paused at the arrest site leaves just enough RNA exposed  to allow binding of SLBP and the U7 snRNP and processing of the transcript.	bind
7313	2	3102	5	11	NULL	0	NULL	statement 1	Process		expose					RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_12_4046_s_279	12773550	(A) RNA polymerase II paused at the arrest site leaves just enough RNA exposed  to allow binding of SLBP and the U7 snRNP and processing of the transcript.	bind
7314	3	3102	5	11	NULL	0	NULL	SLBP	GP		bind					RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_12_4046_s_279	12773550	(A) RNA polymerase II paused at the arrest site leaves just enough RNA exposed  to allow binding of SLBP and the U7 snRNP and processing of the transcript.	bind
7315	4	3102	5	11	NULL	0	NULL	U7 snRNP	NucleicAcid		bind					RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_12_4046_s_279	12773550	(A) RNA polymerase II paused at the arrest site leaves just enough RNA exposed  to allow binding of SLBP and the U7 snRNP and processing of the transcript.	bind
7316	5	3102	5	11	NULL	0	NULL	statement 2	Process		allows					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_12_4046_s_279	12773550	(A) RNA polymerase II paused at the arrest site leaves just enough RNA exposed  to allow binding of SLBP and the U7 snRNP and processing of the transcript.	bind
7317	6	3102	5	11	NULL	0	NULL	statement 2	Process		allows					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_12_4046_s_279	12773550	(A) RNA polymerase II paused at the arrest site leaves just enough RNA exposed  to allow binding of SLBP and the U7 snRNP and processing of the transcript.	bind
7318	7	3102	5	11	NULL	0	NULL	statement 2	Process		allows					transcript	NucleicAcid	processing of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_12_4046_s_279	12773550	(A) RNA polymerase II paused at the arrest site leaves just enough RNA exposed  to allow binding of SLBP and the U7 snRNP and processing of the transcript.	bind
9142	1	3102	7	11	NULL	0	NULL	SLBP	GP		bind					RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_12_4046_s_279	12773550	(A) RNA polymerase II paused at the arrest site leaves just enough RNA exposed  to allow binding of SLBP and the U7 snRNP and processing of the transcript.	bind
9143	2	3102	7	11	NULL	0	NULL	U7 snRNP	NucleicAcid		bind					RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_12_4046_s_279	12773550	(A) RNA polymerase II paused at the arrest site leaves just enough RNA exposed  to allow binding of SLBP and the U7 snRNP and processing of the transcript.	bind
9144	3	3102	7	11	NULL	0	NULL	RNA polymerase II	GP		pause at					arrest site	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_12_4046_s_279	12773550	(A) RNA polymerase II paused at the arrest site leaves just enough RNA exposed  to allow binding of SLBP and the U7 snRNP and processing of the transcript.	bind
9145	4	3102	7	11	NULL	0	NULL	statement 3	Process		allows					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_12_4046_s_279	12773550	(A) RNA polymerase II paused at the arrest site leaves just enough RNA exposed  to allow binding of SLBP and the U7 snRNP and processing of the transcript.	bind
9146	5	3102	7	11	NULL	0	NULL	statement 3	Process		allows					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_12_4046_s_279	12773550	(A) RNA polymerase II paused at the arrest site leaves just enough RNA exposed  to allow binding of SLBP and the U7 snRNP and processing of the transcript.	bind
54165	7	3102	7	11	NULL	0	NULL	statement 3	Process		allows					transcript	NucleicAcid	processing of 			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_12_4046_s_279	12773550	(A) RNA polymerase II paused at the arrest site leaves just enough RNA exposed  to allow binding of SLBP and the U7 snRNP and processing of the transcript.	bind
79248	1	3102	11	NULL	NULL	0	NULL	 RNA polymerase II	GeneOrProtein		paused at the					arrest site	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_12_4046_s_279	12773550	(A) RNA polymerase II paused at the arrest site leaves just enough RNA exposed  to allow binding of SLBP and the U7 snRNP and processing of the transcript.	bind
79249	2	3102	11	NULL	NULL	0	NULL	SLBP	GeneOrProtein		binds					RNA	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_12_4046_s_279	12773550	(A) RNA polymerase II paused at the arrest site leaves just enough RNA exposed  to allow binding of SLBP and the U7 snRNP and processing of the transcript.	bind
79250	3	3102	11	NULL	NULL	0	NULL	 U7 snRNP	NucleicAcidSubstance		binds					RNA	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_12_4046_s_279	12773550	(A) RNA polymerase II paused at the arrest site leaves just enough RNA exposed  to allow binding of SLBP and the U7 snRNP and processing of the transcript.	bind
79251	4	3102	11	NULL	NULL	0	NULL	statement 1	Process		minimize exposure for 					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_12_4046_s_279	12773550	(A) RNA polymerase II paused at the arrest site leaves just enough RNA exposed  to allow binding of SLBP and the U7 snRNP and processing of the transcript.	bind
79252	5	3102	11	NULL	NULL	0	NULL	statement 2	Process		minimize exposure for 					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_12_4046_s_279	12773550	(A) RNA polymerase II paused at the arrest site leaves just enough RNA exposed  to allow binding of SLBP and the U7 snRNP and processing of the transcript.	bind
79253	6	3102	11	NULL	NULL	0	NULL	statement 2	Process		occurs along with					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_12_4046_s_279	12773550	(A) RNA polymerase II paused at the arrest site leaves just enough RNA exposed  to allow binding of SLBP and the U7 snRNP and processing of the transcript.	bind
79254	7	3102	11	NULL	NULL	0	NULL	statement 1	Process		is a part of processing					transcript	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_12_4046_s_279	12773550	(A) RNA polymerase II paused at the arrest site leaves just enough RNA exposed  to allow binding of SLBP and the U7 snRNP and processing of the transcript.	bind
79255	8	3102	11	NULL	NULL	0	NULL	statement 2	Process		is a part of processing					transcript	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_12_4046_s_279	12773550	(A) RNA polymerase II paused at the arrest site leaves just enough RNA exposed  to allow binding of SLBP and the U7 snRNP and processing of the transcript.	bind
79256	9	3102	11	NULL	NULL	0	NULL	statement 3	Process		is a part of processing					transcript	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_12_4046_s_279	12773550	(A) RNA polymerase II paused at the arrest site leaves just enough RNA exposed  to allow binding of SLBP and the U7 snRNP and processing of the transcript.	bind
7440	1	3105	5	11	NULL	0	NULL	RNA	NucleicAcid		bind					RRM3	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_98_6_835_s_234	10499800	(A) RNA would favor binding of  RRM3 and then RRM4.	bind
7441	2	3105	5	11	NULL	0	NULL	RNA	NucleicAcid		bind					RRM4	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_98_6_835_s_234	10499800	(A) RNA would favor binding of  RRM3 and then RRM4.	bind
9485	1	3105	7	11	NULL	0	NULL	RRM3	GP		bind					RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_98_6_835_s_234	10499800	(A) RNA would favor binding of  RRM3 and then RRM4.	bind
9486	2	3105	7	11	NULL	0	NULL	RRM4	GP		bind					RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_98_6_835_s_234	10499800	(A) RNA would favor binding of  RRM3 and then RRM4.	bind
79558	1	3105	11	NULL	NULL	0	NULL	RNA	NucleicAcidSubstance		binds to 					RRM3	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_cell_98_6_835_s_234	10499800	(A) RNA would favor binding of  RRM3 and then RRM4.	bind
79559	2	3105	11	NULL	NULL	0	NULL	RNA	NucleicAcidSubstance		binds to 					RRM4	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_cell_98_6_835_s_234	10499800	(A) RNA would favor binding of  RRM3 and then RRM4.	bind
79560	3	3105	11	NULL	NULL	0	NULL	statement 2	Process		occurs after					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_cell_98_6_835_s_234	10499800	(A) RNA would favor binding of  RRM3 and then RRM4.	bind
7443	1	3106	5	11	NULL	0	NULL	Rtn1p	GP		bind					Sec6p 	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_7_3009_s_274	16624861	(A) Rtn1p binds to the Sec6p subunit of the exocyst.	bind
44742	2	3106	5	11	NULL	0	NULL	Sec6p	GP		is a subunit of					exocyst	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_7_3009_s_274	16624861	(A) Rtn1p binds to the Sec6p subunit of the exocyst.	bind
9147	1	3106	7	11	NULL	0	NULL	Rtn1p	GP		bind					Sec6p 	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_7_3009_s_274	16624861	(A) Rtn1p binds to the Sec6p subunit of the exocyst.	bind
44743	2	3106	7	11	NULL	0	NULL	Sec6p	GP		is a subunit of					exocyst	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_7_3009_s_274	16624861	(A) Rtn1p binds to the Sec6p subunit of the exocyst.	bind
79561	1	3106	11	NULL	NULL	0	NULL	Sec6p	GeneOrProtein		is a subunit of					exocyst	CellComponent				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_7_3009_s_274	16624861	(A) Rtn1p binds to the Sec6p subunit of the exocyst.	bind
79562	2	3106	11	NULL	NULL	0	NULL	Rtn1p	GeneOrProtein		binds to 					Sec6p	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_7_3009_s_274	16624861	(A) Rtn1p binds to the Sec6p subunit of the exocyst.	bind
7444	1	3108	5	11	NULL	0	NULL	sAPP695T	GP		bind					HK forms	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1571_3_225_s_245	12090937	(A) sAPP695T binds to HK forms.	bind
9148	1	3108	7	11	NULL	0	NULL	sAPP695T	GP		bind					HK forms	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1571_3_225_s_245	12090937	(A) sAPP695T binds to HK forms.	bind
79563	1	3108	11	NULL	NULL	0	NULL	sAPP695T	GeneOrProtein		binds to 					HK	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1571_3_225_s_245	12090937	(A) sAPP695T binds to HK forms.	bind
7445	1	3109	5	11	NULL	0	NULL	[125]DTX	Chemical		bind					Kv1.2	GP				NULL	transfected COS1 cells	NULL	NULL	NULL	NULL	gw60_neuron_16_4_843_s_150	8608002	(A) Saturable binding of [125]DTX to Kv1.2 in transfected COS1 cells.	bind
9149	1	3109	7	11	NULL	0	NULL	[125]DTX	Chemical		bind					Kv1.2	GP				NULL	transfected COS1 cells	NULL	NULL	NULL	NULL	gw60_neuron_16_4_843_s_150	8608002	(A) Saturable binding of [125]DTX to Kv1.2 in transfected COS1 cells.	bind
79564	1	3109	11	NULL	NULL	0	NULL	[125]DTX	Chemical		Saturably binds to					Kv1.2	GeneOrProtein	in transfected COS1 cells			NULL		0	NULL	NULL	NULL	gw60_neuron_16_4_843_s_150	8608002	(A) Saturable binding of [125]DTX to Kv1.2 in transfected COS1 cells.	bind
7446	1	3110	5	11	NULL	0	NULL	[3]RX 821002	Chemical		bind					2A AR membrane	CellComponent	wt			NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_42_6_855_s_103	12015212	(A) Saturation binding curve of [3]RX 821002 to wt  2A AR membrane preparation (5  g protein) was performed as described in  Materials and methods.	bind
9150	1	3110	7	11	NULL	0	NULL	[3]RX 821002	Chemical		bind					2A AR membrane	CellComponent	wt			NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_42_6_855_s_103	12015212	(A) Saturation binding curve of [3]RX 821002 to wt  2A AR membrane preparation (5  g protein) was performed as described in  Materials and methods.	bind
7447	1	3111	5	11	NULL	0	NULL	[35]GTP S	Chemical		bind					SPM	CellComponent	mouse;; brain			NULL		NULL	NULL	NULL	NULL	gw60_brainres_815_1_89_s_122	9974126	(A) Saturation binding of [35]GTP S binding to SPM from mouse brain.	bind
9151	1	3111	7	11	NULL	0	NULL	[35]GTP S	Chemical		bind					SPM	CellComponent	mouse;; brain			NULL		NULL	NULL	NULL	NULL	gw60_brainres_815_1_89_s_122	9974126	(A) Saturation binding of [35]GTP S binding to SPM from mouse brain.	bind
79833	1	3111	11	NULL	NULL	NULL	NULL	[35]GTP S	NonProteinOrNucleicAcidChemical		bind		Saturation			SPM	CellComponent	mouse;;brain			NULL		NULL	NULL	NULL	NULL	gw60_brainres_815_1_89_s_122	9974126	(A) Saturation binding of [35]GTP S binding to SPM from mouse brain.	bind
7448	1	3112	5	11	NULL	0	NULL	[3]P4	Chemical		bind					DPR	GP		LBD		NULL		NULL	NULL	NULL	NULL	gw60_febslett_465_1_12_s_161	10620698	(a) Scatchard analysis of [3]P4 and [3]17 ,20 -DP binding to the DPR-LBD.	bind
7449	2	3112	5	11	NULL	0	NULL	[3]17 ,20 -D	Chemical		bind					DPR	GP		LBD		NULL		NULL	NULL	NULL	NULL	gw60_febslett_465_1_12_s_161	10620698	(a) Scatchard analysis of [3]P4 and [3]17 ,20 -DP binding to the DPR-LBD.	bind
9152	1	3112	7	11	NULL	0	NULL	[3]P4	Chemical		bind					DPR	GP		LBD		NULL		NULL	NULL	NULL	NULL	gw60_febslett_465_1_12_s_161	10620698	(a) Scatchard analysis of [3]P4 and [3]17 ,20 -DP binding to the DPR-LBD.	bind
9153	2	3112	7	11	NULL	0	NULL	[3]17 ,20 -DP	Chemical		bind					DPR	GP		LBD		NULL		NULL	NULL	NULL	NULL	gw60_febslett_465_1_12_s_161	10620698	(a) Scatchard analysis of [3]P4 and [3]17 ,20 -DP binding to the DPR-LBD.	bind
79834	1	3112	11	NULL	NULL	0	NULL	17 ,20 -DP	NonProteinOrNucleicAcidChemical		binds to 					DPR-LBD	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_febslett_465_1_12_s_161	10620698	(a) Scatchard analysis of [3]P4 and [3]17 ,20 -DP binding to the DPR-LBD.	bind
79835	2	3112	11	NULL	NULL	NULL	NULL	P4	NonProteinOrNucleicAcidChemical		binds to 					DPR-LBD	GeneOrProtein				NULL		NULL	NULL	NULL	NULL	gw60_febslett_465_1_12_s_161	10620698	(a) Scatchard analysis of [3]P4 and [3]17 ,20 -DP binding to the DPR-LBD.	bind
7450	1	3114	5	11	NULL	0	NULL	Mnk2a	GP		bind					MAPK	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_16_5692_s_474	12897141	(A) Schematic  presentation of Mnk2a bound to MAP kinase (MAPK).	bind
7451	2	3114	5	11	NULL	0	NULL	MAPK	GP		is					MAP kinase	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_16_5692_s_474	12897141	(A) Schematic  presentation of Mnk2a bound to MAP kinase (MAPK).	bind
9154	1	3114	7	11	NULL	0	NULL	Mnk2a 	GP		bind					MAP kinase	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_16_5692_s_474	12897141	(A) Schematic  presentation of Mnk2a bound to MAP kinase (MAPK).	bind
9155	2	3114	7	11	NULL	0	NULL	MAP kinase	GP		is					MAPK	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_16_5692_s_474	12897141	(A) Schematic  presentation of Mnk2a bound to MAP kinase (MAPK).	bind
79565	1	3114	11	NULL	NULL	0	NULL	Mnk2a	GeneOrProtein		binds to 					MAP kinase	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_16_5692_s_474	12897141	(A) Schematic  presentation of Mnk2a bound to MAP kinase (MAPK).	bind
7452	1	3116	5	11	NULL	0	NULL	amphiphysin protein	GP		bind			NH2-terminal domain		lipid bilayers	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_45_6_787_s_120	14529717	(A) Schematic cartoon of the amphiphysin primary  protein sequence showing the highly conserved NH2-terminal domain known to bind and  tubulate lipid bilayers, an internal poly-proline rich region just upstream of the  clathrin and AP-2 binding sites, and a COOH-terminal SH3 domain.	bind
7453	2	3116	5	11	NULL	0	NULL	amphiphysin protein	GP		tubulate			NH2-terminal region		lipid bilayers	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_45_6_787_s_120	14529717	(A) Schematic cartoon of the amphiphysin primary  protein sequence showing the highly conserved NH2-terminal domain known to bind and  tubulate lipid bilayers, an internal poly-proline rich region just upstream of the  clathrin and AP-2 binding sites, and a COOH-terminal SH3 domain.	bind
9487	1	3116	7	11	NULL	0	NULL	amphiphysin	GP		bind			conserved NH2-terminal		lipid bilayer	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_45_6_787_s_120	14529717	(A) Schematic cartoon of the amphiphysin primary  protein sequence showing the highly conserved NH2-terminal domain known to bind and  tubulate lipid bilayers, an internal poly-proline rich region just upstream of the  clathrin and AP-2 binding sites, and a COOH-terminal SH3 domain.	bind
9488	2	3116	7	11	NULL	0	NULL	amphiphysin	GP		tubulate			conserved NH2-terminal		lipid bilayer	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_45_6_787_s_120	14529717	(A) Schematic cartoon of the amphiphysin primary  protein sequence showing the highly conserved NH2-terminal domain known to bind and  tubulate lipid bilayers, an internal poly-proline rich region just upstream of the  clathrin and AP-2 binding sites, and a COOH-terminal SH3 domain.	bind
79836	1	3116	11	NULL	NULL	0	NULL	amphiphysin	Protein		has								NH2-terminal domain		NULL		0	NULL	NULL	NULL	gw70_neuropharmacology_45_6_787_s_120	14529717	(A) Schematic cartoon of the amphiphysin primary  protein sequence showing the highly conserved NH2-terminal domain known to bind and  tubulate lipid bilayers, an internal poly-proline rich region just upstream of the  clathrin and AP-2 binding sites, and a COOH-terminal SH3 domain.	bind
79837	2	3116	11	NULL	NULL	0	NULL	amphiphysin 	Protein		bind			 NH2-terminal domain		lipid bilayers	CellComponent				NULL		0	NULL	NULL	NULL	gw70_neuropharmacology_45_6_787_s_120	14529717	(A) Schematic cartoon of the amphiphysin primary  protein sequence showing the highly conserved NH2-terminal domain known to bind and  tubulate lipid bilayers, an internal poly-proline rich region just upstream of the  clathrin and AP-2 binding sites, and a COOH-terminal SH3 domain.	bind
79838	3	3116	11	NULL	NULL	0	NULL	amphiphysin	Protein		tubulate			 NH2-terminal domain		lipid bilayers	CellComponent				NULL		0	NULL	NULL	NULL	gw70_neuropharmacology_45_6_787_s_120	14529717	(A) Schematic cartoon of the amphiphysin primary  protein sequence showing the highly conserved NH2-terminal domain known to bind and  tubulate lipid bilayers, an internal poly-proline rich region just upstream of the  clathrin and AP-2 binding sites, and a COOH-terminal SH3 domain.	bind
79839	4	3116	11	NULL	NULL	0	NULL	statement 2	Process		occurs along with					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_neuropharmacology_45_6_787_s_120	14529717	(A) Schematic cartoon of the amphiphysin primary  protein sequence showing the highly conserved NH2-terminal domain known to bind and  tubulate lipid bilayers, an internal poly-proline rich region just upstream of the  clathrin and AP-2 binding sites, and a COOH-terminal SH3 domain.	bind
79840	5	3116	11	NULL	NULL	0	NULL	amphiphysin	Protein		has								COOH-terminal SH3 domain		NULL		0	NULL	NULL	NULL	gw70_neuropharmacology_45_6_787_s_120	14529717	(A) Schematic cartoon of the amphiphysin primary  protein sequence showing the highly conserved NH2-terminal domain known to bind and  tubulate lipid bilayers, an internal poly-proline rich region just upstream of the  clathrin and AP-2 binding sites, and a COOH-terminal SH3 domain.	bind
79841	6	3116	11	NULL	NULL	0	NULL	amphiphysin	Protein		has binding site for					clathrin	Protein				NULL		0	NULL	NULL	NULL	gw70_neuropharmacology_45_6_787_s_120	14529717	(A) Schematic cartoon of the amphiphysin primary  protein sequence showing the highly conserved NH2-terminal domain known to bind and  tubulate lipid bilayers, an internal poly-proline rich region just upstream of the  clathrin and AP-2 binding sites, and a COOH-terminal SH3 domain.	bind
79842	7	3116	11	NULL	NULL	0	NULL	amphiphysin	Protein		has binding site for					AP-2	Protein				NULL		0	NULL	NULL	NULL	gw70_neuropharmacology_45_6_787_s_120	14529717	(A) Schematic cartoon of the amphiphysin primary  protein sequence showing the highly conserved NH2-terminal domain known to bind and  tubulate lipid bilayers, an internal poly-proline rich region just upstream of the  clathrin and AP-2 binding sites, and a COOH-terminal SH3 domain.	bind
7454	1	3117	5	NULL	NULL	NULL	NULL	trp	GP		bind				repressor	trp	GP			operator	NULL		NULL	NULL	NULL	NULL	gw60_structure_3_7_635_s_56	8591039	(a) Schematic diagram of the  trp repressor binding to the 20 base-pair  trp operator DNA showing the potential primary and secondary binding modes.	bind
9156	1	3117	7	10	NULL	0	NULL	trp repressor	GP		bind					DNA	NucleicAcid			trp operator	NULL		NULL	NULL	NULL	NULL	gw60_structure_3_7_635_s_56	8591039	(a) Schematic diagram of the  trp repressor binding to the 20 base-pair  trp operator DNA showing the potential primary and secondary binding modes.	bind
79843	1	3117	11	NULL	NULL	NULL	NULL	trp repressor	GeneOrProtein		binds to 					trp operator DNA	NucleicAcidSubstance			20 base-pair	NULL		NULL	NULL	NULL	NULL	gw60_structure_3_7_635_s_56	8591039	(a) Schematic diagram of the  trp repressor binding to the 20 base-pair  trp operator DNA showing the potential primary and secondary binding modes.	bind
7455	1	3119	5	11	NULL	0	NULL	importin	GP	full-length	bind								IBB domain		NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_6_1345_s_117	12504010	(A) Schematic model of full-length importin   bound to both IBB domain and PTHrP-ncNLS.	bind
7456	2	3119	5	11	NULL	0	NULL	importin	GP	full-length	bind					PTHrP	GP		ncNLS		NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_6_1345_s_117	12504010	(A) Schematic model of full-length importin   bound to both IBB domain and PTHrP-ncNLS.	bind
9157	1	3119	7	11	NULL	0	NULL	importin	GP	full-length	bind								IBB domain		NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_6_1345_s_117	12504010	(A) Schematic model of full-length importin   bound to both IBB domain and PTHrP-ncNLS.	bind
9158	2	3119	7	11	NULL	0	NULL	importin	GP	full-length	bind					PTHrP	GP		ncNLS		NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_6_1345_s_117	12504010	(A) Schematic model of full-length importin   bound to both IBB domain and PTHrP-ncNLS.	bind
79844	1	3119	11	NULL	NULL	0	NULL	importin	Protein		binds to 								IBB domain		NULL		0	NULL	NULL	NULL	gw60_molcell_10_6_1345_s_117	12504010	(A) Schematic model of full-length importin   bound to both IBB domain and PTHrP-ncNLS.	bind
79845	2	3119	11	NULL	NULL	0	NULL	importin	Protein		binds to 					PTHrP-ncNLS.	Protein				NULL		0	NULL	NULL	NULL	gw60_molcell_10_6_1345_s_117	12504010	(A) Schematic model of full-length importin   bound to both IBB domain and PTHrP-ncNLS.	bind
7459	1	3123	5	11	NULL	0	NULL	Che-1	GP		bind					Tau	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_24_4_1038_s_84	14697667	(A) Schematic representation  of myc-Che-1 constructs used to identify portions of Che-1 that bind Tau.	bind
9159	1	3123	7	11	NULL	0	NULL	Che-1 	GP		bind					Tau	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_24_4_1038_s_84	14697667	(A) Schematic representation  of myc-Che-1 constructs used to identify portions of Che-1 that bind Tau.	bind
79846	1	3123	11	NULL	NULL	0	NULL	Che-1	Protein		binds to 					Tau	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellneurosci_24_4_1038_s_84	14697667	(A) Schematic representation  of myc-Che-1 constructs used to identify portions of Che-1 that bind Tau.	bind
7460	1	3124	5	11	NULL	0	NULL	myc-Tau	GP		bind					Che-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_24_4_1038_s_72	14697667	(A) Schematic representation  of myc-Tau constructs used to identify the portion of Tau that binds Che-1.	bind
9160	1	3124	7	11	NULL	0	NULL	myc-Tau	GP		bind					Che-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_24_4_1038_s_72	14697667	(A) Schematic representation  of myc-Tau constructs used to identify the portion of Tau that binds Che-1.	bind
79847	1	3124	11	NULL	NULL	0	NULL	Tau	Protein		binds to 					Che-1	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellneurosci_24_4_1038_s_72	14697667	(A) Schematic representation  of myc-Tau constructs used to identify the portion of Tau that binds Che-1.	bind
79757	1	3125	11	NULL	NULL	NULL	NULL	TAP tag	PartOfProtein		composed of 					protein A	Protein				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_9_3519_s_256	15831458	(A) Schematic representation of  CKIP-1 with an amino-terminal TAP tag that is composed of protein A and a calmodulin  binding peptide separated by a TEV cleavage site.	bind
79758	2	3125	11	NULL	NULL	0	NULL	TAP tag	PartOfProtein		composed of 					 calmodulin binding peptide	PartOfProtein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_9_3519_s_256	15831458	(A) Schematic representation of  CKIP-1 with an amino-terminal TAP tag that is composed of protein A and a calmodulin  binding peptide separated by a TEV cleavage site.	bind
79759	3	3125	11	NULL	NULL	NULL	NULL	protein A	Protein		occurs along with					calmodulin binding peptide	PartOfProtein				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_9_3519_s_256	15831458	(A) Schematic representation of  CKIP-1 with an amino-terminal TAP tag that is composed of protein A and a calmodulin  binding peptide separated by a TEV cleavage site.	bind
79849	4	3125	11	NULL	NULL	0	NULL	CKIP-1	Protein		has								 amino-terminal TAP		NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_9_3519_s_256	15831458	(A) Schematic representation of  CKIP-1 with an amino-terminal TAP tag that is composed of protein A and a calmodulin  binding peptide separated by a TEV cleavage site.	bind
7461	1	3126	5	11	NULL	0	NULL	Axin	GP		bind			RGS domain		APC	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_4_3_407_s_142	12636921	(A) Schematic representation of Axin (not to scale) indicating the RGS domain that binds APC, the binding domains for Zw3/Sgg kinase and Armadillo, and the DIX dimerization domain.	bind
9161	1	3126	7	11	NULL	0	NULL	Axin	GP		bind			RGS domain		APC	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_4_3_407_s_142	12636921	(A) Schematic representation of Axin (not to scale) indicating the RGS domain that binds APC, the binding domains for Zw3/Sgg kinase and Armadillo, and the DIX dimerization domain.	bind
79831	1	3126	11	NULL	NULL	NULL	NULL	Axin	Protein		binds			RGS		APC					NULL		NULL	NULL	NULL	NULL	gw60_devcell_4_3_407_s_142	12636921	(A) Schematic representation of Axin (not to scale) indicating the RGS domain that binds APC, the binding domains for Zw3/Sgg kinase and Armadillo, and the DIX dimerization domain.	bind
79853	3	3126	11	NULL	NULL	0	NULL	Axin	Protein		has binding domain for					Zw3/Sgg kinase	Protein				NULL		0	NULL	NULL	NULL	gw60_devcell_4_3_407_s_142	12636921	(A) Schematic representation of Axin (not to scale) indicating the RGS domain that binds APC, the binding domains for Zw3/Sgg kinase and Armadillo, and the DIX dimerization domain.	bind
79855	4	3126	11	NULL	NULL	0	NULL	Axin	Protein		has binding domain for					Armadillo	Protein				NULL		0	NULL	NULL	NULL	gw60_devcell_4_3_407_s_142	12636921	(A) Schematic representation of Axin (not to scale) indicating the RGS domain that binds APC, the binding domains for Zw3/Sgg kinase and Armadillo, and the DIX dimerization domain.	bind
79856	5	3126	11	NULL	NULL	NULL	NULL	Axin	Protein		has 					DIX			dimerization domain		NULL		NULL	NULL	NULL	NULL	gw60_devcell_4_3_407_s_142	12636921	(A) Schematic representation of Axin (not to scale) indicating the RGS domain that binds APC, the binding domains for Zw3/Sgg kinase and Armadillo, and the DIX dimerization domain.	bind
7465	1	3128	5	11	NULL	0	NULL	Raichu-RalA	GP		bind					GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_6_2549_s_54	15034142	(A) Schematic representation of Raichu-RalA bound  to GDP or GTP.	bind
7466	2	3128	5	11	NULL	0	NULL	Raichu-RalA	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_6_2549_s_54	15034142	(A) Schematic representation of Raichu-RalA bound  to GDP or GTP.	bind
7467	3	3128	5	11	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_6_2549_s_54	15034142	(A) Schematic representation of Raichu-RalA bound  to GDP or GTP.	bind
9165	1	3128	7	11	NULL	0	NULL	Raichu-RalA	GP		bind					GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_6_2549_s_54	15034142	(A) Schematic representation of Raichu-RalA bound  to GDP or GTP.	bind
9166	2	3128	7	11	NULL	0	NULL	Raichu-RalA	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_6_2549_s_54	15034142	(A) Schematic representation of Raichu-RalA bound  to GDP or GTP.	bind
11922	3	3128	7	11	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_6_2549_s_54	15034142	(A) Schematic representation of Raichu-RalA bound  to GDP or GTP.	bind
79857	1	3128	11	NULL	NULL	NULL	NULL	Raichu-RalA	GeneOrProtein		binds to 					GDP	NonProteinOrNucleicAcidChemical				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_6_2549_s_54	15034142	(A) Schematic representation of Raichu-RalA bound  to GDP or GTP.	bind
79858	2	3128	11	NULL	NULL	NULL	NULL	Raichu-RalA	GeneOrProtein		binds to 					GTP	NonProteinOrNucleicAcidChemical				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_6_2549_s_54	15034142	(A) Schematic representation of Raichu-RalA bound  to GDP or GTP.	bind
79760	1	3130	11	NULL	NULL	NULL	NULL	 IMD2 sequence	Gene		contain					 NSE region	NucleicAcidSubstance				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_17_6279_s_79	12917348	(A) Schematic representation of the  IMD2 sequence in the NSE region and comparison with the consensus binding elements of  Gcr1p and Abf1p.	bind
7468	1	3132	5	11	NULL	0	NULL	liver transcription factors	GP		bind					HNF-3	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_mechdev_89_1_185_s_13	10559496	(A) Schematic representation of the liver transcription factors binding to the HNF-3   promoter region.	bind
9167	1	3132	7	11	NULL	0	NULL	liver transcription factors	GP		binds to					HNF-3	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_mechdev_89_1_185_s_13	10559496	(A) Schematic representation of the liver transcription factors binding to the HNF-3   promoter region.	bind
79859	1	3132	11	NULL	NULL	NULL	NULL	liver transcription factor	Protein		binds to 					HNF-3	Gene			promoter region	NULL		NULL	NULL	NULL	NULL	gw60_mechdev_89_1_185_s_13	10559496	(A) Schematic representation of the liver transcription factors binding to the HNF-3   promoter region.	bind
7469	1	3136	5	11	NULL	0	NULL	Raichu-Rac	GP		bind					GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6582_s_62	12192056	(A) Schematic representations of Raichu-Rac and Raichu-Cdc42 bound to GDP or GTP.	bind
7470	2	3136	5	11	NULL	0	NULL	Raichu-Rac	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6582_s_62	12192056	(A) Schematic representations of Raichu-Rac and Raichu-Cdc42 bound to GDP or GTP.	bind
7471	3	3136	5	11	NULL	0	NULL	Raichu-Cdc42	GP		bind					GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6582_s_62	12192056	(A) Schematic representations of Raichu-Rac and Raichu-Cdc42 bound to GDP or GTP.	bind
7472	4	3136	5	11	NULL	0	NULL	Raichu-Cdc42	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6582_s_62	12192056	(A) Schematic representations of Raichu-Rac and Raichu-Cdc42 bound to GDP or GTP.	bind
7473	5	3136	5	11	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6582_s_62	12192056	(A) Schematic representations of Raichu-Rac and Raichu-Cdc42 bound to GDP or GTP.	bind
7474	6	3136	5	11	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6582_s_62	12192056	(A) Schematic representations of Raichu-Rac and Raichu-Cdc42 bound to GDP or GTP.	bind
9168	1	3136	7	11	NULL	0	NULL	Raichu-Rac	GP		bind					GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6582_s_62	12192056	(A) Schematic representations of Raichu-Rac and Raichu-Cdc42 bound to GDP or GTP.	bind
9169	2	3136	7	11	NULL	0	NULL	Raichu-Rac	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6582_s_62	12192056	(A) Schematic representations of Raichu-Rac and Raichu-Cdc42 bound to GDP or GTP.	bind
9170	3	3136	7	11	NULL	0	NULL	Raichu-Cdc42	GP		bind					GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6582_s_62	12192056	(A) Schematic representations of Raichu-Rac and Raichu-Cdc42 bound to GDP or GTP.	bind
9171	4	3136	7	11	NULL	0	NULL	Raichu-Cdc42	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6582_s_62	12192056	(A) Schematic representations of Raichu-Rac and Raichu-Cdc42 bound to GDP or GTP.	bind
11923	5	3136	7	11	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6582_s_62	12192056	(A) Schematic representations of Raichu-Rac and Raichu-Cdc42 bound to GDP or GTP.	bind
11924	6	3136	7	11	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6582_s_62	12192056	(A) Schematic representations of Raichu-Rac and Raichu-Cdc42 bound to GDP or GTP.	bind
79863	1	3136	11	NULL	NULL	NULL	NULL	Raichu-Rac	GeneOrProtein		binds to 					GDP	NonProteinOrNucleicAcidChemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6582_s_62	12192056	(A) Schematic representations of Raichu-Rac and Raichu-Cdc42 bound to GDP or GTP.	bind
79864	2	3136	11	NULL	NULL	NULL	NULL	Raichu-Rac	GeneOrProtein		binds to 					GTP	NonProteinOrNucleicAcidChemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6582_s_62	12192056	(A) Schematic representations of Raichu-Rac and Raichu-Cdc42 bound to GDP or GTP.	bind
79865	3	3136	11	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_18_6582_s_62	12192056	(A) Schematic representations of Raichu-Rac and Raichu-Cdc42 bound to GDP or GTP.	bind
79866	4	3136	11	NULL	NULL	NULL	NULL	Raichu-Cdc42	GeneOrProtein		binds to 					GDP	NonProteinOrNucleicAcidChemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6582_s_62	12192056	(A) Schematic representations of Raichu-Rac and Raichu-Cdc42 bound to GDP or GTP.	bind
79867	5	3136	11	NULL	NULL	NULL	NULL	Raichu-Cdc42	GeneOrProtein		binds to 					GTP	NonProteinOrNucleicAcidChemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6582_s_62	12192056	(A) Schematic representations of Raichu-Rac and Raichu-Cdc42 bound to GDP or GTP.	bind
79868	6	3136	11	NULL	NULL	0	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_18_6582_s_62	12192056	(A) Schematic representations of Raichu-Rac and Raichu-Cdc42 bound to GDP or GTP.	bind
7475	1	3137	5	11	NULL	0	NULL	Raichu-RhoA	GP		bind					GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_162_2_223_s_43	12860967	(A) Schematic representations of Raichu-RhoA bound to GDP or GTP.	bind
7476	2	3137	5	11	NULL	0	NULL	Raichu-RhoA	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_162_2_223_s_43	12860967	(A) Schematic representations of Raichu-RhoA bound to GDP or GTP.	bind
7477	3	3137	5	11	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_162_2_223_s_43	12860967	(A) Schematic representations of Raichu-RhoA bound to GDP or GTP.	bind
9172	1	3137	7	11	NULL	0	NULL	Raichu-RhoA	GP		bind					GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_162_2_223_s_43	12860967	(A) Schematic representations of Raichu-RhoA bound to GDP or GTP.	bind
9173	2	3137	7	11	NULL	0	NULL	Raichu-RhoA	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_162_2_223_s_43	12860967	(A) Schematic representations of Raichu-RhoA bound to GDP or GTP.	bind
61115	3	3137	7	11	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_162_2_223_s_43	12860967	(A) Schematic representations of Raichu-RhoA bound to GDP or GTP.	bind
79869	1	3137	11	NULL	NULL	NULL	NULL	Raichu-RhoA	GeneOrProtein		binds to 					GDP	NonProteinOrNucleicAcidChemical				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_162_2_223_s_43	12860967	(A) Schematic representations of Raichu-RhoA bound to GDP or GTP.	bind
79870	2	3137	11	NULL	NULL	NULL	NULL	Raichu-RhoA	GeneOrProtein		binds to 					GTP	NonProteinOrNucleicAcidChemical				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_162_2_223_s_43	12860967	(A) Schematic representations of Raichu-RhoA bound to GDP or GTP.	bind
79871	3	3137	11	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_162_2_223_s_43	12860967	(A) Schematic representations of Raichu-RhoA bound to GDP or GTP.	bind
7478	1	3141	5	11	NULL	0	NULL	NS1 protein	GP		bind					PABII	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_8_2273_s_275	10205180	(A) sequence is blocked by the binding of the NS1 protein to PABII, resulting in the nuclear accumulation of cleaved pre-mRNAs containing short poly	bind
7481	2	3141	5	11	NULL	0	NULL	statement 1	Process		results in					pre-mRNA	NucleicAcid	nuclear accumulation of			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_8_2273_s_275	10205180	(A) sequence is blocked by the binding of the NS1 protein to PABII, resulting in the nuclear accumulation of cleaved pre-mRNAs containing short poly	bind
9278	1	3141	7	11	NULL	0	NULL	NS1	GP		bind					PABII	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_8_2273_s_275	10205180	(A) sequence is blocked by the binding of the NS1 protein to PABII, resulting in the nuclear accumulation of cleaved pre-mRNAs containing short poly	bind
9279	2	3141	7	11	NULL	0	NULL	statement 1	Process		result in					cleaved pre-mRNA	NucleicAcid	nuclear accumulation of			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_8_2273_s_275	10205180	(A) sequence is blocked by the binding of the NS1 protein to PABII, resulting in the nuclear accumulation of cleaved pre-mRNAs containing short poly	bind
79872	1	3141	11	NULL	NULL	NULL	NULL	NS1 protein	Protein		binds to 					PABII	GeneOrProtein				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_8_2273_s_275	10205180	(A) sequence is blocked by the binding of the NS1 protein to PABII, resulting in the nuclear accumulation of cleaved pre-mRNAs containing short poly	bind
79873	2	3141	11	NULL	NULL	NULL	NULL	statement 1	Process		accumulate		nuclear			pre-mRNAs	NucleicAcidSubstance	cleaved			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_8_2273_s_275	10205180	(A) sequence is blocked by the binding of the NS1 protein to PABII, resulting in the nuclear accumulation of cleaved pre-mRNAs containing short poly	bind
79876	1	3142	11	NULL	NULL	0	NULL	tendamistat	Protein		has binding site for					amylase	Protein				NULL		0	NULL	NULL	NULL	gw60_chembiol_10_1_53_s_47	12573698	(A) Sequence of a peptide Ten(15-23) derived from  -amylase binding site of tendamistat  [17]  .	bind
79877	2	3142	11	NULL	NULL	0	NULL	Ten peptide	PartOfProtein		derived from					 tendamistat	Protein		amylase binding site		NULL		0	NULL	NULL	NULL	gw60_chembiol_10_1_53_s_47	12573698	(A) Sequence of a peptide Ten(15-23) derived from  -amylase binding site of tendamistat  [17]  .	bind
79878	1	3144	11	NULL	NULL	NULL	NULL	Phyl	GeneOrProtein		has binding site for					Sina	GeneOrProtein				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_19_6854_s_360	12215542	(A) Sequence of the Sina-binding region of Phyl from residues 109 to 127.	bind
7490	1	3146	5	11	NULL	0	NULL	p53 proteins	GP		bind		sequence specific			DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1517_3_392_s_94	11342217	(A) Sequence-specific DNA binding of various p53 proteins.	bind
9280	1	3146	7	11	NULL	0	NULL	p53 protein	GP		bind		sequence-specific			DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1517_3_392_s_94	11342217	(A) Sequence-specific DNA binding of various p53 proteins.	bind
79879	1	3146	11	NULL	NULL	0	NULL	p53 protein	Protein		binds to 		Sequence-specific			DNA	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1517_3_392_s_94	11342217	(A) Sequence-specific DNA binding of various p53 proteins.	bind
7491	1	3147	5	11	NULL	0	NULL	enolase	GP	A. hydrophila	bind					plasminogen	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_microbpathogenesis_34_4_195_s_117	12668143	(A) showing  A. hydrophila enolase binding to human plasminogen.	bind
9281	1	3147	7	11	NULL	0	NULL	 enolase	GP	A. hydrophila	bind					plasminogen	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_microbpathogenesis_34_4_195_s_117	12668143	(A) showing  A. hydrophila enolase binding to human plasminogen.	bind
79881	1	3147	11	NULL	NULL	NULL	NULL	enolase	Protein	A. hydrophila	binds to 					plasminogen	Protein	human			NULL		NULL	NULL	NULL	NULL	gw60_microbpathogenesis_34_4_195_s_117	12668143	(A) showing  A. hydrophila enolase binding to human plasminogen.	bind
7495	1	3148	5	11	NULL	0	NULL	SFA	Chemical		bind			cyclic region		cyclophilin	GP				NULL		NULL	NULL	NULL	NULL	gw70_febslett_555_2_335_s_120	14644438	(A) shows CsA  [ 33] and (B) shows macrolide 16 [ 32], an analogue of SFA s cyclic region that binds to the cyclophilin, bound to the  active site of human cyclophilin A. Images were produced using Protein Explorer [  34] with the contact surface between the protein and ligand predicted and points of  theoretical contact marked by the rings.	bind
7592	2	3148	5	11	NULL	0	NULL	macrolide 16	Chemical		is an analogue of					SFA	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_febslett_555_2_335_s_120	14644438	(A) shows CsA  [ 33] and (B) shows macrolide 16 [ 32], an analogue of SFA s cyclic region that binds to the cyclophilin, bound to the  active site of human cyclophilin A. Images were produced using Protein Explorer [  34] with the contact surface between the protein and ligand predicted and points of  theoretical contact marked by the rings.	bind
7593	3	3148	5	11	NULL	0	NULL	macrolide 16	Chemical		bind					cyclophilin A	GP	human	active site		NULL		NULL	NULL	NULL	NULL	gw70_febslett_555_2_335_s_120	14644438	(A) shows CsA  [ 33] and (B) shows macrolide 16 [ 32], an analogue of SFA s cyclic region that binds to the cyclophilin, bound to the  active site of human cyclophilin A. Images were produced using Protein Explorer [  34] with the contact surface between the protein and ligand predicted and points of  theoretical contact marked by the rings.	bind
7594	4	3148	5	11	NULL	0	NULL	CsA	Chemical		bind					cyclophilin A	GP	human	active site		NULL		NULL	NULL	NULL	NULL	gw70_febslett_555_2_335_s_120	14644438	(A) shows CsA  [ 33] and (B) shows macrolide 16 [ 32], an analogue of SFA s cyclic region that binds to the cyclophilin, bound to the  active site of human cyclophilin A. Images were produced using Protein Explorer [  34] with the contact surface between the protein and ligand predicted and points of  theoretical contact marked by the rings.	bind
9282	1	3148	7	11	NULL	0	NULL	SFA	Chemical		bind			cyclic region		cyclophilinA	GP				NULL		NULL	NULL	NULL	NULL	gw70_febslett_555_2_335_s_120	14644438	(A) shows CsA  [ 33] and (B) shows macrolide 16 [ 32], an analogue of SFA s cyclic region that binds to the cyclophilin, bound to the  active site of human cyclophilin A. Images were produced using Protein Explorer [  34] with the contact surface between the protein and ligand predicted and points of  theoretical contact marked by the rings.	bind
11926	2	3148	7	11	NULL	0	NULL	CsA	Chemical		bind					cyclophilinA	GP	human	active site 		NULL		NULL	NULL	NULL	NULL	gw70_febslett_555_2_335_s_120	14644438	(A) shows CsA  [ 33] and (B) shows macrolide 16 [ 32], an analogue of SFA s cyclic region that binds to the cyclophilin, bound to the  active site of human cyclophilin A. Images were produced using Protein Explorer [  34] with the contact surface between the protein and ligand predicted and points of  theoretical contact marked by the rings.	bind
11927	3	3148	7	11	NULL	0	NULL	 macrolide 16	Chemical		bind					cyclophilinA	GP	human	active site		NULL		NULL	NULL	NULL	NULL	gw70_febslett_555_2_335_s_120	14644438	(A) shows CsA  [ 33] and (B) shows macrolide 16 [ 32], an analogue of SFA s cyclic region that binds to the cyclophilin, bound to the  active site of human cyclophilin A. Images were produced using Protein Explorer [  34] with the contact surface between the protein and ligand predicted and points of  theoretical contact marked by the rings.	bind
11928	4	3148	7	11	NULL	0	NULL	 macrolide 16	Chemical		is an analogue of					SFA	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_febslett_555_2_335_s_120	14644438	(A) shows CsA  [ 33] and (B) shows macrolide 16 [ 32], an analogue of SFA s cyclic region that binds to the cyclophilin, bound to the  active site of human cyclophilin A. Images were produced using Protein Explorer [  34] with the contact surface between the protein and ligand predicted and points of  theoretical contact marked by the rings.	bind
79882	1	3148	11	NULL	NULL	NULL	NULL	macrolide 16	NonProteinOrNucleicAcidChemical		is an analogue of					SFA	NonProteinOrNucleicAcidChemical	cyclic region			NULL		NULL	NULL	NULL	NULL	gw70_febslett_555_2_335_s_120	14644438	(A) shows CsA  [ 33] and (B) shows macrolide 16 [ 32], an analogue of SFA s cyclic region that binds to the cyclophilin, bound to the  active site of human cyclophilin A. Images were produced using Protein Explorer [  34] with the contact surface between the protein and ligand predicted and points of  theoretical contact marked by the rings.	bind
79883	2	3148	11	NULL	NULL	NULL	NULL	SFA	NonProteinOrNucleicAcidChemical	 cyclic region	binds to 					cyclophilin	Protein				NULL		NULL	NULL	NULL	NULL	gw70_febslett_555_2_335_s_120	14644438	(A) shows CsA  [ 33] and (B) shows macrolide 16 [ 32], an analogue of SFA s cyclic region that binds to the cyclophilin, bound to the  active site of human cyclophilin A. Images were produced using Protein Explorer [  34] with the contact surface between the protein and ligand predicted and points of  theoretical contact marked by the rings.	bind
79884	3	3148	11	NULL	NULL	NULL	NULL	CsA	NonProteinOrNucleicAcidChemical		binds to 					cyclophilin A	Protein	human			NULL		NULL	NULL	NULL	NULL	gw70_febslett_555_2_335_s_120	14644438	(A) shows CsA  [ 33] and (B) shows macrolide 16 [ 32], an analogue of SFA s cyclic region that binds to the cyclophilin, bound to the  active site of human cyclophilin A. Images were produced using Protein Explorer [  34] with the contact surface between the protein and ligand predicted and points of  theoretical contact marked by the rings.	bind
79885	4	3148	11	NULL	NULL	NULL	NULL	macrolide 16	NonProteinOrNucleicAcidChemical		binds to 					cyclophilin A	Protein	human			NULL		NULL	NULL	NULL	NULL	gw70_febslett_555_2_335_s_120	14644438	(A) shows CsA  [ 33] and (B) shows macrolide 16 [ 32], an analogue of SFA s cyclic region that binds to the cyclophilin, bound to the  active site of human cyclophilin A. Images were produced using Protein Explorer [  34] with the contact surface between the protein and ligand predicted and points of  theoretical contact marked by the rings.	bind
7595	1	3151	5	11	NULL	0	NULL	virus	Organism	signal of	bind		effectively			GTFs	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_3_834_s_44	10629040	(A) signal of the virus binds GTFs effectively in a manner characteristic of a promoter.	bind
7596	2	3151	5	11	NULL	0	NULL	statement 1	Process		occurs in manner							characteristic of		promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_3_834_s_44	10629040	(A) signal of the virus binds GTFs effectively in a manner characteristic of a promoter.	bind
9283	1	3151	7	11	NULL	0	NULL	virus	Organism	signal of	bind		effectively			GTFs	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_3_834_s_44	10629040	(A) signal of the virus binds GTFs effectively in a manner characteristic of a promoter.	bind
11929	2	3151	7	11	NULL	0	NULL	statement 1	Process		occurs in a manner					promoter	NucleicAcid	characteristic of 			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_3_834_s_44	10629040	(A) signal of the virus binds GTFs effectively in a manner characteristic of a promoter.	bind
79886	1	3151	11	NULL	NULL	NULL	NULL	 signal	MolecularProcess	 virus	binds to 					GTFs	Gene			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_3_834_s_44	10629040	(A) signal of the virus binds GTFs effectively in a manner characteristic of a promoter.	bind
7597	1	3152	5	11	NULL	0	NULL			upstream	interact with				polypyrimidine tract	polypyrimidine tract binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_376_s_282	9858561	(A) signal, there is an upstream polypyrimidine tract which has been shown to interact both with polypyrimidine tract binding protein and with CstF, which binds cooperatively with CPSF ( 19a).	bind
7598	2	3152	5	11	NULL	0	NULL			upstream	bind				polypyrimidine tract	CstF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_376_s_282	9858561	(A) signal, there is an upstream polypyrimidine tract which has been shown to interact both with polypyrimidine tract binding protein and with CstF, which binds cooperatively with CPSF ( 19a).	bind
7599	3	3152	5	11	NULL	0	NULL	CstF	GP		bind					CPSF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_376_s_282	9858561	(A) signal, there is an upstream polypyrimidine tract which has been shown to interact both with polypyrimidine tract binding protein and with CstF, which binds cooperatively with CPSF ( 19a).	bind
7600	4	3152	5	11	NULL	0	NULL	polypyrimidine tract binding protein	GP		bind					CPSF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_376_s_282	9858561	(A) signal, there is an upstream polypyrimidine tract which has been shown to interact both with polypyrimidine tract binding protein and with CstF, which binds cooperatively with CPSF ( 19a).	bind
7601	5	3152	5	11	NULL	0	NULL	statement 3	Process		occurs in cooperation with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_376_s_282	9858561	(A) signal, there is an upstream polypyrimidine tract which has been shown to interact both with polypyrimidine tract binding protein and with CstF, which binds cooperatively with CPSF ( 19a).	bind
9284	1	3152	7	11	NULL	0	NULL			upstream	bind				polypyrimidine tract	polypyrimidine tract binding protein 	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_376_s_282	9858561	(A) signal, there is an upstream polypyrimidine tract which has been shown to interact both with polypyrimidine tract binding protein and with CstF, which binds cooperatively with CPSF ( 19a).	bind
9285	2	3152	7	11	NULL	0	NULL			upstream	bind				polypyrimidine tract	CstF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_376_s_282	9858561	(A) signal, there is an upstream polypyrimidine tract which has been shown to interact both with polypyrimidine tract binding protein and with CstF, which binds cooperatively with CPSF ( 19a).	bind
9286	3	3152	7	11	NULL	0	NULL	polypyrimidine tract binding protein	GP		bind					CPSF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_376_s_282	9858561	(A) signal, there is an upstream polypyrimidine tract which has been shown to interact both with polypyrimidine tract binding protein and with CstF, which binds cooperatively with CPSF ( 19a).	bind
9287	4	3152	7	11	NULL	0	NULL	CstF	GP		bind					CPSF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_376_s_282	9858561	(A) signal, there is an upstream polypyrimidine tract which has been shown to interact both with polypyrimidine tract binding protein and with CstF, which binds cooperatively with CPSF ( 19a).	bind
11931	5	3152	7	11	NULL	0	NULL	statement 3	Process		occurs in cooperation with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_376_s_282	9858561	(A) signal, there is an upstream polypyrimidine tract which has been shown to interact both with polypyrimidine tract binding protein and with CstF, which binds cooperatively with CPSF ( 19a).	bind
79889	1	3152	11	NULL	NULL	0	NULL	polypyrimidine tract	NucleicAcidSubstance		interact with					polypyrimidine tract binding protein	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_1_376_s_282	9858561	(A) signal, there is an upstream polypyrimidine tract which has been shown to interact both with polypyrimidine tract binding protein and with CstF, which binds cooperatively with CPSF ( 19a).	bind
79890	2	3152	11	NULL	NULL	0	NULL	polypyrimidine tract	NucleicAcidSubstance		interact with					CstF	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_1_376_s_282	9858561	(A) signal, there is an upstream polypyrimidine tract which has been shown to interact both with polypyrimidine tract binding protein and with CstF, which binds cooperatively with CPSF ( 19a).	bind
79891	3	3152	11	NULL	NULL	0	NULL	statement 1	Process		occurs along with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_1_376_s_282	9858561	(A) signal, there is an upstream polypyrimidine tract which has been shown to interact both with polypyrimidine tract binding protein and with CstF, which binds cooperatively with CPSF ( 19a).	bind
79892	4	3152	11	NULL	NULL	0	NULL	CstF	Protein		binds to 		cooperatively			CPSF	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_1_376_s_282	9858561	(A) signal, there is an upstream polypyrimidine tract which has been shown to interact both with polypyrimidine tract binding protein and with CstF, which binds cooperatively with CPSF ( 19a).	bind
7602	1	3153	5	11	NULL	0	NULL	CPSF	GP		bind					RNAs	NucleicAcid	pre-wt			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2660_s_224	10733568	(A) signal, we used electrophoretic mobility shift assays to examine the stability of CPSF binding to the pre-wt and pre-Sp RNAs.	bind
7603	2	3153	5	11	NULL	0	NULL	CPSF	GP		bind					RNAs	NucleicAcid	pre-Sp			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2660_s_224	10733568	(A) signal, we used electrophoretic mobility shift assays to examine the stability of CPSF binding to the pre-wt and pre-Sp RNAs.	bind
9288	1	3153	7	11	NULL	0	NULL	CPSF	GP		bind					RNA	NucleicAcid	pre-wt			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2660_s_224	10733568	(A) signal, we used electrophoretic mobility shift assays to examine the stability of CPSF binding to the pre-wt and pre-Sp RNAs.	bind
9289	2	3153	7	11	NULL	0	NULL	CPSF	GP		bind					RNA	NucleicAcid	pre-Sp			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2660_s_224	10733568	(A) signal, we used electrophoretic mobility shift assays to examine the stability of CPSF binding to the pre-wt and pre-Sp RNAs.	bind
79894	1	3153	11	NULL	NULL	NULL	NULL	CPSF	Protein		binds to 					RNAs	NucleicAcidSubstance	pre-Sp 			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2660_s_224	10733568	(A) signal, we used electrophoretic mobility shift assays to examine the stability of CPSF binding to the pre-wt and pre-Sp RNAs.	bind
79895	2	3153	11	NULL	NULL	NULL	NULL	CPSF	Protein		binds to 					RNAs	NucleicAcidSubstance	pre-wt 			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2660_s_224	10733568	(A) signal, we used electrophoretic mobility shift assays to examine the stability of CPSF binding to the pre-wt and pre-Sp RNAs.	bind
79896	3	3153	11	NULL	NULL	0	NULL	electrophoretic mobility shift assays	ResearchActivity		examine the stability of					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_8_2660_s_224	10733568	(A) signal, we used electrophoretic mobility shift assays to examine the stability of CPSF binding to the pre-wt and pre-Sp RNAs.	bind
79897	4	3153	11	NULL	NULL	0	NULL	electrophoretic mobility shift assays	ResearchActivity		examine the stability of					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_8_2660_s_224	10733568	(A) signal, we used electrophoretic mobility shift assays to examine the stability of CPSF binding to the pre-wt and pre-Sp RNAs.	bind
79950	1	3154	11	NULL	NULL	0	NULL	CPSF	GeneOrProtein		has binding site for					RNA	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_genesdev_17_11_1321_s_114	12782649	(A) signals in the RNA  by the RNA-binding components of CPSF and CstF, and/or by  phosphorylation/dephosphorylation of key components.	bind
79951	2	3154	11	NULL	NULL	0	NULL	CstF	GeneOrProtein		has binding site for					RNA	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_genesdev_17_11_1321_s_114	12782649	(A) signals in the RNA  by the RNA-binding components of CPSF and CstF, and/or by  phosphorylation/dephosphorylation of key components.	bind
7604	1	3155	5	11	NULL	0	NULL	AP-ES	GP		bind					CPAE cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_4_811_s_109	11336704	(A) Significant reduction of AP-ES binding to CPAE cells is seen after pre-treatment with sodium chlorate and 100 nM of Heparinase I, III, or I+II+III, as compared to untreated cells.	bind
7605	2	3155	5	11	NULL	0	NULL	statement 1	Process		reduced by		significantly			sodium chlorate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_4_811_s_109	11336704	(A) Significant reduction of AP-ES binding to CPAE cells is seen after pre-treatment with sodium chlorate and 100 nM of Heparinase I, III, or I+II+III, as compared to untreated cells.	bind
7606	3	3155	5	11	NULL	0	NULL	statement 1	Process		reduced by		significantly			Heparinase I	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_4_811_s_109	11336704	(A) Significant reduction of AP-ES binding to CPAE cells is seen after pre-treatment with sodium chlorate and 100 nM of Heparinase I, III, or I+II+III, as compared to untreated cells.	bind
7607	4	3155	5	11	NULL	0	NULL	statement 1	Process		reduced by		significantly			Heparinase III	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_4_811_s_109	11336704	(A) Significant reduction of AP-ES binding to CPAE cells is seen after pre-treatment with sodium chlorate and 100 nM of Heparinase I, III, or I+II+III, as compared to untreated cells.	bind
7608	5	3155	5	11	NULL	0	NULL	statement 1	Process		reduced by		significantly			Heparinase I+II+III	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_4_811_s_109	11336704	(A) Significant reduction of AP-ES binding to CPAE cells is seen after pre-treatment with sodium chlorate and 100 nM of Heparinase I, III, or I+II+III, as compared to untreated cells.	bind
9290	1	3155	7	11	NULL	0	NULL	AP-ES	GP		bind					CPAE cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_4_811_s_109	11336704	(A) Significant reduction of AP-ES binding to CPAE cells is seen after pre-treatment with sodium chlorate and 100 nM of Heparinase I, III, or I+II+III, as compared to untreated cells.	bind
9291	2	3155	7	11	NULL	0	NULL	statement 1	Process		 reduced by		significantly			sodium chlorate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_4_811_s_109	11336704	(A) Significant reduction of AP-ES binding to CPAE cells is seen after pre-treatment with sodium chlorate and 100 nM of Heparinase I, III, or I+II+III, as compared to untreated cells.	bind
9292	3	3155	7	11	NULL	0	NULL	statement 1	Process		 reduced by		significantly			Heparinase I	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_4_811_s_109	11336704	(A) Significant reduction of AP-ES binding to CPAE cells is seen after pre-treatment with sodium chlorate and 100 nM of Heparinase I, III, or I+II+III, as compared to untreated cells.	bind
9293	4	3155	7	11	NULL	0	NULL	statement 1	Process		 reduced by		significantly			Heparinase I+II+III	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_4_811_s_109	11336704	(A) Significant reduction of AP-ES binding to CPAE cells is seen after pre-treatment with sodium chlorate and 100 nM of Heparinase I, III, or I+II+III, as compared to untreated cells.	bind
9294	5	3155	7	11	NULL	0	NULL	statement 1	Process		reduced by		significantly			Heparinase III	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_4_811_s_109	11336704	(A) Significant reduction of AP-ES binding to CPAE cells is seen after pre-treatment with sodium chlorate and 100 nM of Heparinase I, III, or I+II+III, as compared to untreated cells.	bind
79952	1	3155	11	NULL	NULL	NULL	NULL	AP-ES	GeneOrProtein		binds to 					CPAE cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_4_811_s_109	11336704	(A) Significant reduction of AP-ES binding to CPAE cells is seen after pre-treatment with sodium chlorate and 100 nM of Heparinase I, III, or I+II+III, as compared to untreated cells.	bind
79953	2	3155	11	NULL	NULL	NULL	NULL	sodium chlorate	NonProteinOrNucleicAcidChemical	pre-treatment	reduces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_4_811_s_109	11336704	(A) Significant reduction of AP-ES binding to CPAE cells is seen after pre-treatment with sodium chlorate and 100 nM of Heparinase I, III, or I+II+III, as compared to untreated cells.	bind
79954	3	3155	11	NULL	NULL	0	NULL	Heparinase I	Protein		reduces					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_7_4_811_s_109	11336704	(A) Significant reduction of AP-ES binding to CPAE cells is seen after pre-treatment with sodium chlorate and 100 nM of Heparinase I, III, or I+II+III, as compared to untreated cells.	bind
79955	4	3155	11	NULL	NULL	0	NULL	Heparinase III	Protein		reduces					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_7_4_811_s_109	11336704	(A) Significant reduction of AP-ES binding to CPAE cells is seen after pre-treatment with sodium chlorate and 100 nM of Heparinase I, III, or I+II+III, as compared to untreated cells.	bind
79956	5	3155	11	NULL	NULL	0	NULL	Heparinase II	Protein		reduces					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_7_4_811_s_109	11336704	(A) Significant reduction of AP-ES binding to CPAE cells is seen after pre-treatment with sodium chlorate and 100 nM of Heparinase I, III, or I+II+III, as compared to untreated cells.	bind
79957	6	3155	11	NULL	NULL	0	NULL	statement 3	Process		occurs along with					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_7_4_811_s_109	11336704	(A) Significant reduction of AP-ES binding to CPAE cells is seen after pre-treatment with sodium chlorate and 100 nM of Heparinase I, III, or I+II+III, as compared to untreated cells.	bind
79958	7	3155	11	NULL	NULL	0	NULL	statement 3	Process		occurs along with					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_7_4_811_s_109	11336704	(A) Significant reduction of AP-ES binding to CPAE cells is seen after pre-treatment with sodium chlorate and 100 nM of Heparinase I, III, or I+II+III, as compared to untreated cells.	bind
79959	8	3155	11	NULL	NULL	0	NULL	statement 4	Process		occurs along with					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_7_4_811_s_109	11336704	(A) Significant reduction of AP-ES binding to CPAE cells is seen after pre-treatment with sodium chlorate and 100 nM of Heparinase I, III, or I+II+III, as compared to untreated cells.	bind
7615	1	3156	5	11	NULL	0	NULL	MIWI	GP		bind					oligo(dT)	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_36_13415_s_86	16938833	(A) significantly reduces both MIWI and MSY2 binding in both RNP and polysome fractions, indicating that MIWI binds oligo(dT) through associated poly	bind
9298	1	3156	7	11	NULL	0	NULL	MIWI	GP		bind					oligo(dT)	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_36_13415_s_86	16938833	(A) significantly reduces both MIWI and MSY2 binding in both RNP and polysome fractions, indicating that MIWI binds oligo(dT) through associated poly	bind
79960	1	3156	11	NULL	NULL	0	NULL	MIWI 	Protein		binds to 					oligo(dT)	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_pnas_103_36_13415_s_86	16938833	(A) significantly reduces both MIWI and MSY2 binding in both RNP and polysome fractions, indicating that MIWI binds oligo(dT) through associated poly	bind
79961	1	3157	11	NULL	NULL	NULL	NULL	ZZ-WT Op18	NucleicAcidSubstance		binds to 					IgG Sepharose	Protein				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_153_1_149_s_107	11285281	(A) Silver-stained gel of MgCl2 elutions of control, ZZ-WT, -AAA, and -EEE Op18 bound to IgG Sepharose retrieved from extracts.	bind
79962	2	3157	11	NULL	NULL	NULL	NULL	ZZ-AAA Op18	NucleicAcidSubstance		binds to 					IgG Sepharose	Protein				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_153_1_149_s_107	11285281	(A) Silver-stained gel of MgCl2 elutions of control, ZZ-WT, -AAA, and -EEE Op18 bound to IgG Sepharose retrieved from extracts.	bind
79963	3	3157	11	NULL	NULL	NULL	NULL	ZZ-EEE Op18	NucleicAcidSubstance		binds to 					IgG Sepharose	Protein				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_153_1_149_s_107	11285281	(A) Silver-stained gel of MgCl2 elutions of control, ZZ-WT, -AAA, and -EEE Op18 bound to IgG Sepharose retrieved from extracts.	bind
7616	1	3158	5	11	NULL	0	NULL	CstF	GP		is					cleavage stimulation factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_23_6603_s_31	12456666	(A) site also requires cleavage stimulation factor (CstF) that binds to a GU/U-rich element downstream of the cleavage site and interacts with CPSF.	bind
7617	2	3158	5	11	NULL	0	NULL				lies downstream of				GU/U-rich element	cleavage site	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_23_6603_s_31	12456666	(A) site also requires cleavage stimulation factor (CstF) that binds to a GU/U-rich element downstream of the cleavage site and interacts with CPSF.	bind
7618	3	3158	5	11	NULL	0	NULL	CstF	GP		interact with					CPSF	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_23_6603_s_31	12456666	(A) site also requires cleavage stimulation factor (CstF) that binds to a GU/U-rich element downstream of the cleavage site and interacts with CPSF.	bind
44745	4	3158	5	11	NULL	0	NULL	CstF	GP		bind					statement 2	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_23_6603_s_31	12456666	(A) site also requires cleavage stimulation factor (CstF) that binds to a GU/U-rich element downstream of the cleavage site and interacts with CPSF.	bind
9299	1	3158	7	11	NULL	0	NULL				lies downstream of				GU/U-rich element	clevage site	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_23_6603_s_31	12456666	(A) site also requires cleavage stimulation factor (CstF) that binds to a GU/U-rich element downstream of the cleavage site and interacts with CPSF.	bind
9300	2	3158	7	11	NULL	0	NULL	statement 1	NucleicAcid		binds					CPSF	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_23_6603_s_31	12456666	(A) site also requires cleavage stimulation factor (CstF) that binds to a GU/U-rich element downstream of the cleavage site and interacts with CPSF.	bind
9301	3	3158	7	11	NULL	0	NULL	cleavage stimulation factor 	GP		is					CstF	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_23_6603_s_31	12456666	(A) site also requires cleavage stimulation factor (CstF) that binds to a GU/U-rich element downstream of the cleavage site and interacts with CPSF.	bind
44746	4	3158	7	11	NULL	0	NULL	CstF	GP		bind					statement 1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_23_6603_s_31	12456666	(A) site also requires cleavage stimulation factor (CstF) that binds to a GU/U-rich element downstream of the cleavage site and interacts with CPSF.	bind
79964	1	3158	11	NULL	NULL	0	NULL	cleavage stimulation factor	Protein		is					CstF	Protein				NULL		0	NULL	NULL	NULL	gw60_embo_21_23_6603_s_31	12456666	(A) site also requires cleavage stimulation factor (CstF) that binds to a GU/U-rich element downstream of the cleavage site and interacts with CPSF.	bind
79965	2	3158	11	NULL	NULL	0	NULL	CstF	Protein		binds to 									GU/U-rich element	NULL		0	NULL	NULL	NULL	gw60_embo_21_23_6603_s_31	12456666	(A) site also requires cleavage stimulation factor (CstF) that binds to a GU/U-rich element downstream of the cleavage site and interacts with CPSF.	bind
79966	3	3158	11	NULL	NULL	NULL	NULL	CstF	Protein		interacts with					CPSF	GeneOrProtein				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_23_6603_s_31	12456666	(A) site also requires cleavage stimulation factor (CstF) that binds to a GU/U-rich element downstream of the cleavage site and interacts with CPSF.	bind
7619	1	3159	5	11	NULL	0	NULL	CPSF	GP		bind					pre-mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_41825_s_295	11551915	(A) site are necessary for the predominant use of the L1 site early in infection ( 39,  44), that splice sites are not involved ( 41), and that binding of CPSF to the pre-mRNA is stabilized by these regulatory sequences ( 53).	bind
7620	2	3159	5	11	NULL	0	NULL				stabilize				regulatory sequences	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_41825_s_295	11551915	(A) site are necessary for the predominant use of the L1 site early in infection ( 39,  44), that splice sites are not involved ( 41), and that binding of CPSF to the pre-mRNA is stabilized by these regulatory sequences ( 53).	bind
9302	1	3159	7	11	NULL	0	NULL	CPSF	GP		bind					pre-mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_41825_s_295	11551915	(A) site are necessary for the predominant use of the L1 site early in infection ( 39,  44), that splice sites are not involved ( 41), and that binding of CPSF to the pre-mRNA is stabilized by these regulatory sequences ( 53).	bind
11932	2	3159	7	11	NULL	0	NULL				stabilize				regulatory sequences	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_41825_s_295	11551915	(A) site are necessary for the predominant use of the L1 site early in infection ( 39,  44), that splice sites are not involved ( 41), and that binding of CPSF to the pre-mRNA is stabilized by these regulatory sequences ( 53).	bind
79967	1	3159	11	NULL	NULL	0	NULL	 CPSF	Protein		binds to 					pre-mRNA	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_45_41825_s_295	11551915	(A) site are necessary for the predominant use of the L1 site early in infection ( 39,  44), that splice sites are not involved ( 41), and that binding of CPSF to the pre-mRNA is stabilized by these regulatory sequences ( 53).	bind
79968	2	3159	11	NULL	NULL	0	NULL	statement 1	Process		is stabilized by					regulatory sequences	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_45_41825_s_295	11551915	(A) site are necessary for the predominant use of the L1 site early in infection ( 39,  44), that splice sites are not involved ( 41), and that binding of CPSF to the pre-mRNA is stabilized by these regulatory sequences ( 53).	bind
7621	1	3163	5	11	NULL	0	NULL	CPSF	GP		bind							upstream of cleavage site		A(A/U)UAAA hexamer	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_11_1315_s_5	15937220	(A) site selection appears to rely primarily on the binding of CPSF to an A(A/U)UAAA hexamer upstream of the cleavage site and CstF to a downstream GU-rich element.	bind
7622	2	3163	5	11	NULL	0	NULL	CstF	GP		bind							downstream		GU-rich element	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_11_1315_s_5	15937220	(A) site selection appears to rely primarily on the binding of CPSF to an A(A/U)UAAA hexamer upstream of the cleavage site and CstF to a downstream GU-rich element.	bind
9303	1	3163	7	11	NULL	0	NULL	CPSF	GP		bind							upstream of the cleavage site		A(A/U)UAAA hexamer	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_11_1315_s_5	15937220	(A) site selection appears to rely primarily on the binding of CPSF to an A(A/U)UAAA hexamer upstream of the cleavage site and CstF to a downstream GU-rich element.	bind
9304	2	3163	7	11	NULL	0	NULL	CstF	GP		bind							downstream		 GU-rich element	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_11_1315_s_5	15937220	(A) site selection appears to rely primarily on the binding of CPSF to an A(A/U)UAAA hexamer upstream of the cleavage site and CstF to a downstream GU-rich element.	bind
79969	1	3163	11	NULL	NULL	0	NULL	CPSF	Protein		binds to 									A(A/U)UAAA hexamer	NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1315_s_5	15937220	(A) site selection appears to rely primarily on the binding of CPSF to an A(A/U)UAAA hexamer upstream of the cleavage site and CstF to a downstream GU-rich element.	bind
79970	2	3163	11	NULL	NULL	0	NULL	CstF	Protein		binds to 									GU-rich element	NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1315_s_5	15937220	(A) site selection appears to rely primarily on the binding of CPSF to an A(A/U)UAAA hexamer upstream of the cleavage site and CstF to a downstream GU-rich element.	bind
7623	1	3164	5	11	NULL	0	NULL	CstF-64	GP		bind							downstream		G/U-rich sequence	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_6_1684_s_28	11865048	(A) site, while CstF-64 binds a downstream G/U-rich sequence.	bind
9305	1	3164	7	11	NULL	0	NULL	CstF-64	GP		binds 							downstream		G/U-rich sequence	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_6_1684_s_28	11865048	(A) site, while CstF-64 binds a downstream G/U-rich sequence.	bind
79971	1	3164	11	NULL	NULL	0	NULL	CstF-64	Protein		binds to 									G/U-rich sequence	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_6_1684_s_28	11865048	(A) site, while CstF-64 binds a downstream G/U-rich sequence.	bind
7624	1	3165	5	11	NULL	0	NULL	CPSF	GP		bind					pre-mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_11_1315_s_348	15937220	(A) site-containing RNA, and that CFIm enhanced the binding of CPSF to the pre-mRNA.	bind
7625	2	3165	5	11	NULL	0	NULL	CFIm	GP		enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_11_1315_s_348	15937220	(A) site-containing RNA, and that CFIm enhanced the binding of CPSF to the pre-mRNA.	bind
9306	1	3165	7	11	NULL	0	NULL	CPSF	GP		bind					pre-mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_11_1315_s_348	15937220	(A) site-containing RNA, and that CFIm enhanced the binding of CPSF to the pre-mRNA.	bind
9307	2	3165	7	11	NULL	0	NULL	CFIm 	GP		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_11_1315_s_348	15937220	(A) site-containing RNA, and that CFIm enhanced the binding of CPSF to the pre-mRNA.	bind
79972	1	3165	11	NULL	NULL	0	NULL	CPSF	Protein		binds to 					pre-mRNA	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1315_s_348	15937220	(A) site-containing RNA, and that CFIm enhanced the binding of CPSF to the pre-mRNA.	bind
79973	2	3165	11	NULL	NULL	0	NULL	RNA	NucleicAcidSubstance		enhances					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1315_s_348	15937220	(A) site-containing RNA, and that CFIm enhanced the binding of CPSF to the pre-mRNA.	bind
79974	3	3165	11	NULL	NULL	NULL	NULL	CFIm	GeneOrProtein		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_11_1315_s_348	15937220	(A) site-containing RNA, and that CFIm enhanced the binding of CPSF to the pre-mRNA.	bind
7626	1	3167	5	11	NULL	0	NULL	L3	GP		bind					CstF	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_87_5_779_s_124	8945502	(A) sites have different strengths so that  L3 binds CstF with higher affinity than L1.	bind
7627	2	3167	5	11	NULL	0	NULL	L3	GP		bind					L1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_87_5_779_s_124	8945502	(A) sites have different strengths so that  L3 binds CstF with higher affinity than L1.	bind
7628	3	3167	5	11	NULL	0	NULL	statement 1	Process		has higher affinity than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_87_5_779_s_124	8945502	(A) sites have different strengths so that  L3 binds CstF with higher affinity than L1.	bind
9308	1	3167	7	11	NULL	0	NULL	L3	GP		bind					CstF	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_87_5_779_s_124	8945502	(A) sites have different strengths so that  L3 binds CstF with higher affinity than L1.	bind
9309	2	3167	7	11	NULL	0	NULL	L1	GP		bind					CstF	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_87_5_779_s_124	8945502	(A) sites have different strengths so that  L3 binds CstF with higher affinity than L1.	bind
9310	3	3167	7	11	NULL	0	NULL	statement 1	Process		has higher affinity than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_87_5_779_s_124	8945502	(A) sites have different strengths so that  L3 binds CstF with higher affinity than L1.	bind
79975	1	3167	11	NULL	NULL	0	NULL	L3	NucleicAcidSubstance		binds to 					CstF	Protein				NULL		0	NULL	NULL	NULL	gw60_cell_87_5_779_s_124	8945502	(A) sites have different strengths so that  L3 binds CstF with higher affinity than L1.	bind
79976	2	3167	11	NULL	NULL	0	NULL	L1	NucleicAcidSubstance		binds to 					CstF	Protein				NULL		0	NULL	NULL	NULL	gw60_cell_87_5_779_s_124	8945502	(A) sites have different strengths so that  L3 binds CstF with higher affinity than L1.	bind
79977	3	3167	11	NULL	NULL	0	NULL	statement 1	Process		has more affinity than					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_cell_87_5_779_s_124	8945502	(A) sites have different strengths so that  L3 binds CstF with higher affinity than L1.	bind
7629	1	3168	5	11	NULL	0	NULL	Skp2	GP		interact with					Smad4	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_17_7524_s_74	15314162	(A) Skp2 interacts with Smad4 but not other  Smads.	bind
7630	2	3168	5	11	NULL	0	NULL	Skp2	GP		does not bind					Smads	GP	other			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_17_7524_s_74	15314162	(A) Skp2 interacts with Smad4 but not other  Smads.	bind
9311	1	3168	7	11	NULL	0	NULL	Skp2	GP		binds					Smad4	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_17_7524_s_74	15314162	(A) Skp2 interacts with Smad4 but not other  Smads.	bind
9312	2	3168	7	11	NULL	0	NULL	Skp2	GP		does not bind					Smads	GP	other			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_17_7524_s_74	15314162	(A) Skp2 interacts with Smad4 but not other  Smads.	bind
79978	1	3168	11	NULL	NULL	NULL	NULL	Skp2	GeneOrProtein		interacts with					Smad4	GeneOrProtein				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_17_7524_s_74	15314162	(A) Skp2 interacts with Smad4 but not other  Smads.	bind
7645	1	3169	5	11	NULL	0	NULL	Smad3A	GP		does not bind					PKA 	GP		regulatory subunit		NULL	TGFbeta-treated cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_5_2169_s_177	14966294	(A) Smad3A does not bind to the PKA regulatory subunit in TGFbeta-treated  cells.	bind
9313	1	3169	7	11	NULL	0	NULL	Smad3A	GP		does not bind					PKA	GP		regulatory subunit		NULL	TGFbeta-treated cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_5_2169_s_177	14966294	(A) Smad3A does not bind to the PKA regulatory subunit in TGFbeta-treated  cells.	bind
79979	1	3169	11	NULL	NULL	0	NULL	 Smad3A	GeneOrProtein		does not bind to					PKA	GeneOrProtein			regulatory subunit	NULL	TGFbeta-treated cells	0	NULL	NULL	NULL	gw70_molcellbiol_24_5_2169_s_177	14966294	(A) Smad3A does not bind to the PKA regulatory subunit in TGFbeta-treated  cells.	bind
7643	1	3170	5	11	NULL	0	NULL	Smad7	GP		bind					p38	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molbiolcell_14_2_529_s_242	12589052	(A) Smad7 binds to p38 in vivo.	bind
9314	1	3170	7	11	NULL	0	NULL	Smad7	GP		bind					p38	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molbiolcell_14_2_529_s_242	12589052	(A) Smad7 binds to p38 in vivo.	bind
79980	1	3170	11	NULL	NULL	0	NULL	 Smad7	GeneOrProtein		binds to 					 p38	GeneOrProtein				NULL	in vivo	0	NULL	NULL	NULL	gw60_molbiolcell_14_2_529_s_242	12589052	(A) Smad7 binds to p38 in vivo.	bind
7646	1	3171	5	11	NULL	0	NULL	Smad7	GP		bind			Y211A		TGF receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_6_1365_s_250	11163210	(A) Smad7(Y211A) binds to TGF  receptors but has a reduced ability to recruit Smurf2 to the receptor complex.	bind
7647	2	3171	5	11	NULL	0	NULL	Smurf2	GP		is recruited to					receptor complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_6_1365_s_250	11163210	(A) Smad7(Y211A) binds to TGF  receptors but has a reduced ability to recruit Smurf2 to the receptor complex.	bind
9315	1	3171	7	11	NULL	0	NULL	Smad7	GP		bind			Y211A		TGF receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_6_1365_s_250	11163210	(A) Smad7(Y211A) binds to TGF  receptors but has a reduced ability to recruit Smurf2 to the receptor complex.	bind
9316	2	3171	7	11	NULL	0	NULL	Smurf2	GP		is recruited to					receptor complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_6_1365_s_250	11163210	(A) Smad7(Y211A) binds to TGF  receptors but has a reduced ability to recruit Smurf2 to the receptor complex.	bind
9317	3	3171	7	11	NULL	0	NULL	Smad7	GP		has reduced ability for			Y211A		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_6_1365_s_250	11163210	(A) Smad7(Y211A) binds to TGF  receptors but has a reduced ability to recruit Smurf2 to the receptor complex.	bind
79981	1	3171	11	NULL	NULL	0	NULL	 Smad7	Protein		binds to 			Y211A		TGF receptor	Protein				NULL		0	NULL	NULL	NULL	gw60_molcell_6_6_1365_s_250	11163210	(A) Smad7(Y211A) binds to TGF  receptors but has a reduced ability to recruit Smurf2 to the receptor complex.	bind
79982	2	3171	11	NULL	NULL	NULL	NULL	Smad7	Protein		recruit		reduced ability to	Y211A		Smurf2	GeneOrProtein				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_6_1365_s_250	11163210	(A) Smad7(Y211A) binds to TGF  receptors but has a reduced ability to recruit Smurf2 to the receptor complex.	bind
7648	1	3173	5	11	NULL	0	NULL	H3 peptide	GP		contain							trimethylated	K9		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5535_s_125	15964809	(a) Space-filling  representation of H3 peptide containing trimethylated K9 bound to  Drosophila HP1 chromodomain.	bind
7650	2	3173	5	11	NULL	0	NULL	statement 1	GP		bind					HP1	GP	Drosophila	chromodomain		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5535_s_125	15964809	(a) Space-filling  representation of H3 peptide containing trimethylated K9 bound to  Drosophila HP1 chromodomain.	bind
9318	1	3173	7	11	NULL	0	NULL	H3 peptide	GP		contain							trimethylated	K9		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5535_s_125	15964809	(a) Space-filling  representation of H3 peptide containing trimethylated K9 bound to  Drosophila HP1 chromodomain.	bind
44747	2	3173	7	11	NULL	0	NULL	statement 1	GP		bind					HP1	GP	Drosophila	chromodomain		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5535_s_125	15964809	(a) Space-filling  representation of H3 peptide containing trimethylated K9 bound to  Drosophila HP1 chromodomain.	bind
79983	1	3173	11	NULL	NULL	0	NULL	H3 peptide	PartOfProtein		contains					K9	PartOfProtein	trimethylated			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_13_5535_s_125	15964809	(a) Space-filling  representation of H3 peptide containing trimethylated K9 bound to  Drosophila HP1 chromodomain.	bind
79984	2	3173	11	NULL	NULL	0	NULL	H3 peptide 	PartOfProtein		binds to 			trimethylated K9		HP1 chromodomain	PartOfProtein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_13_5535_s_125	15964809	(a) Space-filling  representation of H3 peptide containing trimethylated K9 bound to  Drosophila HP1 chromodomain.	bind
7654	1	3174	5	11	NULL	0	NULL	SPB	Chromosome		bind					Cdc14p	GP				NULL	cdc15-1 cells	NULL	NULL	NULL	NULL	gw60_cellbiol_157_3_367_s_269	11970961	(A) SPB binding of Cdc14p in  cdc15-1 and  dbf2-2 cells.	bind
7656	2	3174	5	11	NULL	0	NULL	SPB	Chromosome		bind					Cdc14p	GP				NULL	dbf2-2 cells	NULL	NULL	NULL	NULL	gw60_cellbiol_157_3_367_s_269	11970961	(A) SPB binding of Cdc14p in  cdc15-1 and  dbf2-2 cells.	bind
9319	1	3174	7	11	NULL	0	NULL	SPB	Chromosome		bind					Cdc14p	GP				NULL	cdc15-1 cells	NULL	NULL	NULL	NULL	gw60_cellbiol_157_3_367_s_269	11970961	(A) SPB binding of Cdc14p in  cdc15-1 and  dbf2-2 cells.	bind
9320	2	3174	7	11	NULL	0	NULL	SPB	Chromosome		bind					Cdc14p	GP				NULL	dbf2-2 cells	NULL	NULL	NULL	NULL	gw60_cellbiol_157_3_367_s_269	11970961	(A) SPB binding of Cdc14p in  cdc15-1 and  dbf2-2 cells.	bind
79985	1	3174	11	NULL	NULL	0	NULL	Cdc14p	Protein		binds to 					SPB	CellComponent	cdc15-1;;dbf2-2 cells			NULL		0	NULL	NULL	NULL	gw60_cellbiol_157_3_367_s_269	11970961	(A) SPB binding of Cdc14p in  cdc15-1 and  dbf2-2 cells.	bind
7660	1	3176	5	11	NULL	0	NULL	tomosyn	GP		bind		specifically			syntaxin-1a	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_20_5_905_s_72	9620695	(A) Specific binding of tomosyn to syntaxin-1a.	bind
9321	1	3176	7	11	NULL	0	NULL	tomosyn	GP		bind		specifically			syntaxin-1a	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_20_5_905_s_72	9620695	(A) Specific binding of tomosyn to syntaxin-1a.	bind
79986	1	3176	11	NULL	NULL	NULL	NULL	tomosyn	GeneOrProtein		binds to 					syntaxin-1a	GeneOrProtein				NULL		NULL	NULL	NULL	NULL	gw60_neuron_20_5_905_s_72	9620695	(A) Specific binding of tomosyn to syntaxin-1a.	bind
7668	1	3177	5	11	NULL	0	NULL	VHH	GP		bind		specifically	9C		ISP	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1624_1_21_s_83	14642809	(A) Specific binding of VHH 9C with  P. pastoris-produced ISP as determined with surface plasmon resonance using the anti-ISP VHH  immobilized on flow cell 2 and an anti-lipase VHH on flow cell 1.	bind
9322	1	3177	7	11	NULL	0	NULL	VHH	GP		binds		specifically	 9C		ISP	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1624_1_21_s_83	14642809	(A) Specific binding of VHH 9C with  P. pastoris-produced ISP as determined with surface plasmon resonance using the anti-ISP VHH  immobilized on flow cell 2 and an anti-lipase VHH on flow cell 1.	bind
79987	1	3177	11	NULL	NULL	NULL	NULL	VHH 9C	Protein		binds to 					ISP	Protein	P. pastoris			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1624_1_21_s_83	14642809	(A) Specific binding of VHH 9C with  P. pastoris-produced ISP as determined with surface plasmon resonance using the anti-ISP VHH  immobilized on flow cell 2 and an anti-lipase VHH on flow cell 1.	bind
7675	2	3178	5	11	NULL	0	NULL	[3]AII	GP		bind		specifically			statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_8_1495_s_99	12721105	(a) Specific binding of [3]AII to HEK 293 cells stably or transiently expressing AT1R - YFP or to untransfected cells.	bind
7676	4	3178	5	11	NULL	0	NULL	[3]AII	GP		bind		specifically			statement 3	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_8_1495_s_99	12721105	(a) Specific binding of [3]AII to HEK 293 cells stably or transiently expressing AT1R - YFP or to untransfected cells.	bind
7678	5	3178	5	11	NULL	0	NULL	[3]AII	GP		bind		specifically			HEK 293 cells	Cell	untransfected cells			NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_8_1495_s_99	12721105	(a) Specific binding of [3]AII to HEK 293 cells stably or transiently expressing AT1R - YFP or to untransfected cells.	bind
7679	6	3178	5	11	NULL	0	NULL	statement 5	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_8_1495_s_99	12721105	(a) Specific binding of [3]AII to HEK 293 cells stably or transiently expressing AT1R - YFP or to untransfected cells.	bind
7680	7	3178	5	11	NULL	0	NULL	statement 4	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_8_1495_s_99	12721105	(a) Specific binding of [3]AII to HEK 293 cells stably or transiently expressing AT1R - YFP or to untransfected cells.	bind
44759	1	3178	5	11	NULL	0	NULL	HEK 293 cells	Cell		express		stably			AT1R - YFP	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_8_1495_s_99	12721105	(a) Specific binding of [3]AII to HEK 293 cells stably or transiently expressing AT1R - YFP or to untransfected cells.	bind
44760	3	3178	5	11	NULL	0	NULL	HEK 293 cells	Cell		express		transiently			AT1R - YFP	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_8_1495_s_99	12721105	(a) Specific binding of [3]AII to HEK 293 cells stably or transiently expressing AT1R - YFP or to untransfected cells.	bind
9323	3	3178	7	11	NULL	0	NULL	[3]AII	GP		bind		specifically			statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_8_1495_s_99	12721105	(a) Specific binding of [3]AII to HEK 293 cells stably or transiently expressing AT1R - YFP or to untransfected cells.	bind
9324	4	3178	7	11	NULL	0	NULL	[3]AII	GP		bind		specifically			statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_8_1495_s_99	12721105	(a) Specific binding of [3]AII to HEK 293 cells stably or transiently expressing AT1R - YFP or to untransfected cells.	bind
9325	5	3178	7	11	NULL	0	NULL	[3]AII	GP		bind		specifically			HEK 293 cells	Cell	untransfected			NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_8_1495_s_99	12721105	(a) Specific binding of [3]AII to HEK 293 cells stably or transiently expressing AT1R - YFP or to untransfected cells.	bind
11936	6	3178	7	11	NULL	0	NULL	statement 3	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_8_1495_s_99	12721105	(a) Specific binding of [3]AII to HEK 293 cells stably or transiently expressing AT1R - YFP or to untransfected cells.	bind
11937	7	3178	7	11	NULL	0	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_8_1495_s_99	12721105	(a) Specific binding of [3]AII to HEK 293 cells stably or transiently expressing AT1R - YFP or to untransfected cells.	bind
44726	1	3178	7	11	NULL	0	NULL	HEK293 cells	Cell		express		stably			AT1R - YFP	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_8_1495_s_99	12721105	(a) Specific binding of [3]AII to HEK 293 cells stably or transiently expressing AT1R - YFP or to untransfected cells.	bind
44727	2	3178	7	11	NULL	0	NULL	HEK293 cells	Cell		express		transiently			AT1R - YFP	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_8_1495_s_99	12721105	(a) Specific binding of [3]AII to HEK 293 cells stably or transiently expressing AT1R - YFP or to untransfected cells.	bind
79989	1	3178	11	NULL	NULL	NULL	NULL	AII	GeneOrProtein		binds to 		Specific			HEK 293 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_8_1495_s_99	12721105	(a) Specific binding of [3]AII to HEK 293 cells stably or transiently expressing AT1R - YFP or to untransfected cells.	bind
7684	1	3179	5	11	NULL	0	NULL	PPARalpha/RXRalpha	GP		bind		specifically			PEX11alpha/perilipin	GP			PPRE	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_3_1313_s_236	14729975	(A) Specific PPARalpha/RXRalpha binding to the PEX11alpha/perilipin-PPRE.	bind
9326	1	3179	7	11	NULL	0	NULL	PPARalpha/RXRalpha	GP		bind		specifically			PEX11alpha/perilipin	GP			PPRE	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_3_1313_s_236	14729975	(A) Specific PPARalpha/RXRalpha binding to the PEX11alpha/perilipin-PPRE.	bind
79996	1	3179	11	NULL	NULL	NULL	NULL	PPARalpha	GeneOrProtein		complex with 					RXRalpha	GeneOrProtein				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_3_1313_s_236	14729975	(A) Specific PPARalpha/RXRalpha binding to the PEX11alpha/perilipin-PPRE.	bind
79997	2	3179	11	NULL	NULL	NULL	NULL	PEX11alpha	GeneOrProtein		complex with 					perilipin	GeneOrProtein				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_3_1313_s_236	14729975	(A) Specific PPARalpha/RXRalpha binding to the PEX11alpha/perilipin-PPRE.	bind
79998	3	3179	11	NULL	NULL	NULL	NULL	statement 2	GeneOrProtein		complex with 					PPRE	Gene				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_3_1313_s_236	14729975	(A) Specific PPARalpha/RXRalpha binding to the PEX11alpha/perilipin-PPRE.	bind
79999	4	3179	11	NULL	NULL	NULL	NULL	statement 1	GeneOrProtein		binds to 					statement 3	GeneOrProtein				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_3_1313_s_236	14729975	(A) Specific PPARalpha/RXRalpha binding to the PEX11alpha/perilipin-PPRE.	bind
7773	1	3180	5	11	NULL	0	NULL	transferrin	GP		bind		specifically			L5 fusion	GP		Loop 5		NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_2_732_s_217	11796606	(A) Specific transferrin binding to L5 fusion (Loop 5) compared to CBD alone (CBD control).	bind
7774	2	3180	5	11	NULL	0	NULL	transferrin	GP		bind							control	CBD		NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_2_732_s_217	11796606	(A) Specific transferrin binding to L5 fusion (Loop 5) compared to CBD alone (CBD control).	bind
9327	1	3180	7	11	NULL	0	NULL	transferrin	GP		bind		specifically			 L5 fusion	GP		Loop 5		NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_2_732_s_217	11796606	(A) Specific transferrin binding to L5 fusion (Loop 5) compared to CBD alone (CBD control).	bind
9328	2	3180	7	11	NULL	0	NULL	transferrin	GP		bind								CBD		NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_2_732_s_217	11796606	(A) Specific transferrin binding to L5 fusion (Loop 5) compared to CBD alone (CBD control).	bind
80000	1	3180	11	NULL	NULL	0	NULL	 transferrin	Protein		binds to 					 L5 fusion	PartOfProtein		Loop 5		NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_2_732_s_217	11796606	(A) Specific transferrin binding to L5 fusion (Loop 5) compared to CBD alone (CBD control).	bind
80001	2	3180	11	NULL	NULL	0	NULL	transferrin	Protein		binds to 								CBD		NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_2_732_s_217	11796606	(A) Specific transferrin binding to L5 fusion (Loop 5) compared to CBD alone (CBD control).	bind
7772	1	3181	5	11	NULL	0	NULL	SRC-1	GP		bind					UNC-5	GP		cytosolic domain		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_15_6485_s_48	16024786	(A) SRC-1 binds  the UNC-5 cytosolic domain.	bind
9329	1	3181	7	11	NULL	0	NULL	SRC-1	GP		binds					UNC-5	GP		cytosolic domain		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_15_6485_s_48	16024786	(A) SRC-1 binds  the UNC-5 cytosolic domain.	bind
80002	1	3181	11	NULL	NULL	NULL	NULL	SRC-1	GeneOrProtein		binds to 					UNC-5	Protein		cytosolic domain		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_15_6485_s_48	16024786	(A) SRC-1 binds  the UNC-5 cytosolic domain.	bind
7775	1	3182	5	11	NULL	0	NULL	SREBP-1a	GP		bind					LDL receptor	GP	rat		SRE within promoter at 242 to 234 bp	NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1761_4_492_s_167	16647292	(A) SREBP-1a  binding to the SRE identified within the rat LDL receptor promoter at  242 to  234  bp.	bind
9330	1	3182	7	11	NULL	0	NULL	SREBP-1a	GP		binds to					LDL receptor	GP	rat		SRE promoter at 242 to 234 bp	NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1761_4_492_s_167	16647292	(A) SREBP-1a  binding to the SRE identified within the rat LDL receptor promoter at  242 to  234  bp.	bind
80003	1	3182	11	NULL	NULL	NULL	NULL	SREBP-1a	GeneOrProtein		binds to 					 LDL receptor	Gene	rat		promoter	NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1761_4_492_s_167	16647292	(A) SREBP-1a  binding to the SRE identified within the rat LDL receptor promoter at  242 to  234  bp.	bind
80004	2	3182	11	NULL	NULL	NULL	NULL				is a part of				SRE	LDL receptor	Gene			promoter	NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1761_4_492_s_167	16647292	(A) SREBP-1a  binding to the SRE identified within the rat LDL receptor promoter at  242 to  234  bp.	bind
7777	1	3183	5	11	NULL	0	NULL	caspase-7	GP	active	bind					XIAP fragment	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_3_399_s_80	11701129	(A) Stabilization of the catalytic cleft by the  loop-bundle in the active caspase-7 bound with  an XIAP fragment (PDB code 1I51).	bind
7780	2	3183	5	11	NULL	0	NULL	statement 1	Process		stabilize								catalytic cleft		NULL		NULL	NULL	NULL	NULL	gw60_cell_107_3_399_s_80	11701129	(A) Stabilization of the catalytic cleft by the  loop-bundle in the active caspase-7 bound with  an XIAP fragment (PDB code 1I51).	bind
9331	1	3183	7	11	NULL	0	NULL	caspase-7 	GP	active	bind					 XIAP fragment	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_3_399_s_80	11701129	(A) Stabilization of the catalytic cleft by the  loop-bundle in the active caspase-7 bound with  an XIAP fragment (PDB code 1I51).	bind
11939	2	3183	7	11	NULL	0	NULL	statement 1	Process		stabilize								catalytic cleft		NULL		NULL	NULL	NULL	NULL	gw60_cell_107_3_399_s_80	11701129	(A) Stabilization of the catalytic cleft by the  loop-bundle in the active caspase-7 bound with  an XIAP fragment (PDB code 1I51).	bind
80005	1	3183	11	NULL	NULL	NULL	NULL	caspase-7	GeneOrProtein		binds to 					XIAP fragment	PartOfProtein				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_3_399_s_80	11701129	(A) Stabilization of the catalytic cleft by the  loop-bundle in the active caspase-7 bound with  an XIAP fragment (PDB code 1I51).	bind
7784	1	3184	5	11	NULL	0	NULL	Ste12	GP	yeast lysates	bind		specifically			GST-Rst1	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_4_228_s_78	9094309	(a) Ste12 and Fus3 from yeast lysates bind specifically to GST-Rst1 and GST-Rst2 fusion proteins.	bind
7786	2	3184	5	11	NULL	0	NULL	Ste12	GP	yeast lysates	bind		specifically			GST-Rst2	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_4_228_s_78	9094309	(a) Ste12 and Fus3 from yeast lysates bind specifically to GST-Rst1 and GST-Rst2 fusion proteins.	bind
7787	3	3184	5	11	NULL	0	NULL	Fus3	GP	yeast lysates	bind		specifically			GST-Rst1	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_4_228_s_78	9094309	(a) Ste12 and Fus3 from yeast lysates bind specifically to GST-Rst1 and GST-Rst2 fusion proteins.	bind
7788	4	3184	5	11	NULL	0	NULL	Fus3	GP	yeast lysates	bind		specifically			GST-Rst2	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_4_228_s_78	9094309	(a) Ste12 and Fus3 from yeast lysates bind specifically to GST-Rst1 and GST-Rst2 fusion proteins.	bind
9332	1	3184	7	11	NULL	0	NULL	Ste12	GP	 yeast lysates	bind		specifically			GST-Rst1	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_4_228_s_78	9094309	(a) Ste12 and Fus3 from yeast lysates bind specifically to GST-Rst1 and GST-Rst2 fusion proteins.	bind
9333	2	3184	7	11	NULL	0	NULL	Ste12 	GP	yeast lysates	bind		specifically			GST-Rst2	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_4_228_s_78	9094309	(a) Ste12 and Fus3 from yeast lysates bind specifically to GST-Rst1 and GST-Rst2 fusion proteins.	bind
9334	3	3184	7	11	NULL	0	NULL	Fus3	GP	yeast lysates	bind		specifically			GST-Rst1	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_4_228_s_78	9094309	(a) Ste12 and Fus3 from yeast lysates bind specifically to GST-Rst1 and GST-Rst2 fusion proteins.	bind
9335	4	3184	7	11	NULL	0	NULL	Fus3	GP	yeast lysates	bind		specifically			GST-Rst2	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_4_228_s_78	9094309	(a) Ste12 and Fus3 from yeast lysates bind specifically to GST-Rst1 and GST-Rst2 fusion proteins.	bind
80006	1	3184	11	NULL	NULL	NULL	NULL	Ste12	GeneOrProtein	yeast	binds to 		specifically			GST-Rst2 fusion protein	Protein				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_4_228_s_78	9094309	(a) Ste12 and Fus3 from yeast lysates bind specifically to GST-Rst1 and GST-Rst2 fusion proteins.	bind
80007	2	3184	11	NULL	NULL	NULL	NULL	Fus3	GeneOrProtein	yeast	binds to 		specifically			GST-Rst2 fusion protein	Protein				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_4_228_s_78	9094309	(a) Ste12 and Fus3 from yeast lysates bind specifically to GST-Rst1 and GST-Rst2 fusion proteins.	bind
80008	3	3184	11	NULL	NULL	NULL	NULL	Ste12	GeneOrProtein	yeast	binds to 		specifically			GST-Rst1 fusion protein	Protein				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_4_228_s_78	9094309	(a) Ste12 and Fus3 from yeast lysates bind specifically to GST-Rst1 and GST-Rst2 fusion proteins.	bind
80009	4	3184	11	NULL	NULL	NULL	NULL	Fus3	GeneOrProtein	yeast	binds to 		specifically			GST-Rst1 fusion protein	Protein				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_4_228_s_78	9094309	(a) Ste12 and Fus3 from yeast lysates bind specifically to GST-Rst1 and GST-Rst2 fusion proteins.	bind
7789	1	3185	5	11	NULL	0	NULL	STE50	GP		bind		constitutively			STE11	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_10_5788_s_243	9742096	(A) STE50 binds to STE11 in a constitutive manner.	bind
9336	1	3185	7	11	NULL	0	NULL	STE50	GP		binds		constitutively			STE11	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_10_5788_s_243	9742096	(A) STE50 binds to STE11 in a constitutive manner.	bind
80010	1	3185	11	NULL	NULL	NULL	NULL	STE50	GeneOrProtein		binds to 					STE11	GeneOrProtein				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_10_5788_s_243	9742096	(A) STE50 binds to STE11 in a constitutive manner.	bind
9337	1	3187	7	11	NULL	0	NULL	[35]GTP S	Chemical		bind					 5-ht5A/HEK293 membrane	CellComponent	guinea pig			NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_51_3_566_s_195	16846620	(A) Stimulation by 5-HT, 5-CT, ergotamine, LSD and 8-OH-DPAT of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes; (B) 5-HT-induced stimulation of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes in the absence, and presence, of LSD, clozapine, SB-269970-A or  WAY-100635.	bind
9338	2	3187	7	11	NULL	0	NULL	5-HT	GP		induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_51_3_566_s_195	16846620	(A) Stimulation by 5-HT, 5-CT, ergotamine, LSD and 8-OH-DPAT of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes; (B) 5-HT-induced stimulation of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes in the absence, and presence, of LSD, clozapine, SB-269970-A or  WAY-100635.	bind
9339	3	3187	7	11	NULL	0	NULL	5-CT	Chemical		induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_51_3_566_s_195	16846620	(A) Stimulation by 5-HT, 5-CT, ergotamine, LSD and 8-OH-DPAT of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes; (B) 5-HT-induced stimulation of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes in the absence, and presence, of LSD, clozapine, SB-269970-A or  WAY-100635.	bind
9340	4	3187	7	11	NULL	0	NULL	ergotamine	Chemical		induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_51_3_566_s_195	16846620	(A) Stimulation by 5-HT, 5-CT, ergotamine, LSD and 8-OH-DPAT of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes; (B) 5-HT-induced stimulation of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes in the absence, and presence, of LSD, clozapine, SB-269970-A or  WAY-100635.	bind
9341	5	3187	7	11	NULL	0	NULL	LSD	Chemical		induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_51_3_566_s_195	16846620	(A) Stimulation by 5-HT, 5-CT, ergotamine, LSD and 8-OH-DPAT of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes; (B) 5-HT-induced stimulation of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes in the absence, and presence, of LSD, clozapine, SB-269970-A or  WAY-100635.	bind
9342	6	3187	7	11	NULL	0	NULL	8-OH-DPAT	Chemical		induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_51_3_566_s_195	16846620	(A) Stimulation by 5-HT, 5-CT, ergotamine, LSD and 8-OH-DPAT of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes; (B) 5-HT-induced stimulation of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes in the absence, and presence, of LSD, clozapine, SB-269970-A or  WAY-100635.	bind
80012	1	3187	11	NULL	NULL	NULL	NULL	[35]GTP S	NonProteinOrNucleicAcidChemical		binds to 					5-ht5A	GeneOrProtein	HEK293 membrane;;guinea pig			NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_51_3_566_s_195	16846620	(A) Stimulation by 5-HT, 5-CT, ergotamine, LSD and 8-OH-DPAT of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes; (B) 5-HT-induced stimulation of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes in the absence, and presence, of LSD, clozapine, SB-269970-A or  WAY-100635.	bind
80013	2	3187	11	NULL	NULL	NULL	NULL	 5-HT	NonProteinOrNucleicAcidChemical		stimulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_51_3_566_s_195	16846620	(A) Stimulation by 5-HT, 5-CT, ergotamine, LSD and 8-OH-DPAT of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes; (B) 5-HT-induced stimulation of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes in the absence, and presence, of LSD, clozapine, SB-269970-A or  WAY-100635.	bind
80014	3	3187	11	NULL	NULL	NULL	NULL	5-CT	NonProteinOrNucleicAcidChemical		stimulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_51_3_566_s_195	16846620	(A) Stimulation by 5-HT, 5-CT, ergotamine, LSD and 8-OH-DPAT of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes; (B) 5-HT-induced stimulation of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes in the absence, and presence, of LSD, clozapine, SB-269970-A or  WAY-100635.	bind
80015	4	3187	11	NULL	NULL	NULL	NULL	ergotamine	NonProteinOrNucleicAcidChemical		stimulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_51_3_566_s_195	16846620	(A) Stimulation by 5-HT, 5-CT, ergotamine, LSD and 8-OH-DPAT of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes; (B) 5-HT-induced stimulation of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes in the absence, and presence, of LSD, clozapine, SB-269970-A or  WAY-100635.	bind
80016	5	3187	11	NULL	NULL	NULL	NULL	LSD	NonProteinOrNucleicAcidChemical		stimulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_51_3_566_s_195	16846620	(A) Stimulation by 5-HT, 5-CT, ergotamine, LSD and 8-OH-DPAT of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes; (B) 5-HT-induced stimulation of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes in the absence, and presence, of LSD, clozapine, SB-269970-A or  WAY-100635.	bind
80017	6	3187	11	NULL	NULL	NULL	NULL	8-OH-DPAT	NonProteinOrNucleicAcidChemical		stimulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_51_3_566_s_195	16846620	(A) Stimulation by 5-HT, 5-CT, ergotamine, LSD and 8-OH-DPAT of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes; (B) 5-HT-induced stimulation of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes in the absence, and presence, of LSD, clozapine, SB-269970-A or  WAY-100635.	bind
80018	7	3187	11	NULL	NULL	0	NULL	statement 2	Process		is independent of					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_neuropharmacology_51_3_566_s_195	16846620	(A) Stimulation by 5-HT, 5-CT, ergotamine, LSD and 8-OH-DPAT of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes; (B) 5-HT-induced stimulation of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes in the absence, and presence, of LSD, clozapine, SB-269970-A or  WAY-100635.	bind
80019	8	3187	11	NULL	NULL	NULL	NULL	statement 2	Process		is independent of					clozapine	NonProteinOrNucleicAcidChemical				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_51_3_566_s_195	16846620	(A) Stimulation by 5-HT, 5-CT, ergotamine, LSD and 8-OH-DPAT of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes; (B) 5-HT-induced stimulation of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes in the absence, and presence, of LSD, clozapine, SB-269970-A or  WAY-100635.	bind
80020	9	3187	11	NULL	NULL	NULL	NULL	statement 2	Process		is independent of					SB-269970-A	NonProteinOrNucleicAcidChemical				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_51_3_566_s_195	16846620	(A) Stimulation by 5-HT, 5-CT, ergotamine, LSD and 8-OH-DPAT of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes; (B) 5-HT-induced stimulation of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes in the absence, and presence, of LSD, clozapine, SB-269970-A or  WAY-100635.	bind
80021	10	3187	11	NULL	NULL	NULL	NULL	statement 2	Process		is independent of					WAY-100635	NonProteinOrNucleicAcidChemical				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_51_3_566_s_195	16846620	(A) Stimulation by 5-HT, 5-CT, ergotamine, LSD and 8-OH-DPAT of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes; (B) 5-HT-induced stimulation of [35]GTP S binding to guinea pig 5-ht5A/HEK293 membranes in the absence, and presence, of LSD, clozapine, SB-269970-A or  WAY-100635.	bind
7790	1	3188	5	11	NULL	0	NULL	Rac	GP		bind					PAK	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_150_1_205_s_115	10893268	(A) Stimulation of Rac and Cdc42 binding to PAK.	bind
7791	2	3188	5	11	NULL	0	NULL	Cdc42	GP		bind					PAK	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_150_1_205_s_115	10893268	(A) Stimulation of Rac and Cdc42 binding to PAK.	bind
9343	1	3188	7	11	NULL	0	NULL	Rac	GP		bind					PAK	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_150_1_205_s_115	10893268	(A) Stimulation of Rac and Cdc42 binding to PAK.	bind
9344	2	3188	7	11	NULL	0	NULL	Cdc42	GP		bind					PAK	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_150_1_205_s_115	10893268	(A) Stimulation of Rac and Cdc42 binding to PAK.	bind
80022	1	3188	11	NULL	NULL	NULL	NULL	 Rac	GeneOrProtein		binds to 					PAK	GeneOrProtein				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_150_1_205_s_115	10893268	(A) Stimulation of Rac and Cdc42 binding to PAK.	bind
80023	2	3188	11	NULL	NULL	NULL	NULL	Cdc42	GeneOrProtein		binds to 					PAK	GeneOrProtein				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_150_1_205_s_115	10893268	(A) Stimulation of Rac and Cdc42 binding to PAK.	bind
7792	1	3189	5	11	NULL	0	NULL	PABP	GP		bind					adenosine residues	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genomeres_12_9_1333_s_240	12213770	(A) stretches in a cooperative manner, in which one molecule of PABP binds ~25 adenosine residues (Smith et al. 1997  ).	bind
9345	1	3189	7	11	NULL	0	NULL	PABP 	GP		bind					adenosine residues	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genomeres_12_9_1333_s_240	12213770	(A) stretches in a cooperative manner, in which one molecule of PABP binds ~25 adenosine residues (Smith et al. 1997  ).	bind
80027	1	3189	11	NULL	NULL	NULL	NULL	PABP	GeneOrProtein		binds to 					adenosine	NucleicAcidSubstance			~25 residues	NULL		NULL	NULL	NULL	NULL	gw60_genomeres_12_9_1333_s_240	12213770	(A) stretches in a cooperative manner, in which one molecule of PABP binds ~25 adenosine residues (Smith et al. 1997  ).	bind
7793	1	3190	5	11	NULL	0	NULL	BC1 RNAs	NucleicAcid		bind					PABP	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_8_2374_s_280	16682445	(A) stretches of the RNA and could be alleviated by the addition of PABP ( ), suggesting that the suppression is mediated through binding of PABP by BC1 and BC200 RNAs.	bind
7794	2	3190	5	11	NULL	0	NULL	BC200 RNAs	NucleicAcid		bind					PABP	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_8_2374_s_280	16682445	(A) stretches of the RNA and could be alleviated by the addition of PABP ( ), suggesting that the suppression is mediated through binding of PABP by BC1 and BC200 RNAs.	bind
9346	1	3190	7	11	NULL	0	NULL	PABP	GP		bind					BC1 RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_8_2374_s_280	16682445	(A) stretches of the RNA and could be alleviated by the addition of PABP ( ), suggesting that the suppression is mediated through binding of PABP by BC1 and BC200 RNAs.	bind
9347	2	3190	7	11	NULL	0	NULL	PABP	GP		bind					BC200 RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_8_2374_s_280	16682445	(A) stretches of the RNA and could be alleviated by the addition of PABP ( ), suggesting that the suppression is mediated through binding of PABP by BC1 and BC200 RNAs.	bind
80028	1	3190	11	NULL	NULL	NULL	NULL	PABP	GeneOrProtein		alleviate 					RNA	NucleicAcidSubstance	stretches			NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_8_2374_s_280	16682445	(A) stretches of the RNA and could be alleviated by the addition of PABP ( ), suggesting that the suppression is mediated through binding of PABP by BC1 and BC200 RNAs.	bind
80029	2	3190	11	NULL	NULL	NULL	NULL	PABP	GeneOrProtein		binds to 					BC200 RNA	NucleicAcidSubstance				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_8_2374_s_280	16682445	(A) stretches of the RNA and could be alleviated by the addition of PABP ( ), suggesting that the suppression is mediated through binding of PABP by BC1 and BC200 RNAs.	bind
80030	3	3190	11	NULL	NULL	NULL	NULL	PABP	GeneOrProtein		binds to 					BC1 RNA	NucleicAcidSubstance				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_8_2374_s_280	16682445	(A) stretches of the RNA and could be alleviated by the addition of PABP ( ), suggesting that the suppression is mediated through binding of PABP by BC1 and BC200 RNAs.	bind
7795	1	3191	5	11	NULL	0	NULL	RNAP II	GP	S. cerevisiae	bind					nucleic acids	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_70_1_12_s_19	16524917	(A) Structure of  S. cerevisiae RNAP II bound to nucleic acids (PDB accession number 1Y1W).	bind
9348	1	3191	7	11	NULL	0	NULL	RNAP II	GP	S. cerevisiae	bind					nucleic acids	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_70_1_12_s_19	16524917	(A) Structure of  S. cerevisiae RNAP II bound to nucleic acids (PDB accession number 1Y1W).	bind
80031	1	3191	11	NULL	NULL	NULL	NULL	RNAP II	GeneOrProtein	S. cerevisiae	binds to 					nucleic acid	NucleicAcidSubstance				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_70_1_12_s_19	16524917	(A) Structure of  S. cerevisiae RNAP II bound to nucleic acids (PDB accession number 1Y1W).	bind
7796	1	3194	5	11	NULL	0	NULL				bind			tandem SH3 domains		p22 peptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_113_3_343_s_196	12732142	(A) Structure of the tandem SH3 domains bound to the p22 peptide.	bind
9349	1	3194	7	11	NULL	0	NULL				bind			tandem SH3 domains		p22 peptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_113_3_343_s_196	12732142	(A) Structure of the tandem SH3 domains bound to the p22 peptide.	bind
80032	1	3194	11	NULL	NULL	0	NULL				binds to 			SH3 domains		p22 peptide	PartOfProtein				NULL		0	NULL	NULL	NULL	gw60_cell_113_3_343_s_196	12732142	(A) Structure of the tandem SH3 domains bound to the p22 peptide.	bind
7806	1	3196	5	11	NULL	0	NULL	Caf1	GP		bind					chaperone G1	GP	donor strand			NULL		NULL	NULL	NULL	NULL	gw60_cell_113_5_587_s_250	12787500	(A) Superposition of Caf1  (red) bound to the chaperone G1 donor strand (blue) and Caf1  (yellow) bound to the Caf1  Gd donor strand (orange) (stereo view).	bind
7809	2	3196	5	11	NULL	0	NULL	Caf1	GP		bind					Caf1 Gd	GP	donor strand			NULL		NULL	NULL	NULL	NULL	gw60_cell_113_5_587_s_250	12787500	(A) Superposition of Caf1  (red) bound to the chaperone G1 donor strand (blue) and Caf1  (yellow) bound to the Caf1  Gd donor strand (orange) (stereo view).	bind
9350	1	3196	7	11	NULL	0	NULL	Caf1	GP		bind					chaperone G1	GP	donor strand			NULL		NULL	NULL	NULL	NULL	gw60_cell_113_5_587_s_250	12787500	(A) Superposition of Caf1  (red) bound to the chaperone G1 donor strand (blue) and Caf1  (yellow) bound to the Caf1  Gd donor strand (orange) (stereo view).	bind
9351	2	3196	7	11	NULL	0	NULL	Caf1	GP		bind					Caf1 Gd	GP	donor strand			NULL		NULL	NULL	NULL	NULL	gw60_cell_113_5_587_s_250	12787500	(A) Superposition of Caf1  (red) bound to the chaperone G1 donor strand (blue) and Caf1  (yellow) bound to the Caf1  Gd donor strand (orange) (stereo view).	bind
80033	1	3196	11	NULL	NULL	NULL	NULL	Caf1	GeneOrProtein		binds to 					chaperone G1	GeneOrProtein	donor strand			NULL		NULL	NULL	NULL	NULL	gw60_cell_113_5_587_s_250	12787500	(A) Superposition of Caf1  (red) bound to the chaperone G1 donor strand (blue) and Caf1  (yellow) bound to the Caf1  Gd donor strand (orange) (stereo view).	bind
80034	2	3196	11	NULL	NULL	NULL	NULL	Caf1	GeneOrProtein		binds to 					Caf1 Gd	GeneOrProtein	donor strand			NULL		NULL	NULL	NULL	NULL	gw60_cell_113_5_587_s_250	12787500	(A) Superposition of Caf1  (red) bound to the chaperone G1 donor strand (blue) and Caf1  (yellow) bound to the Caf1  Gd donor strand (orange) (stereo view).	bind
8194	1	3197	5	11	NULL	0	NULL	TSL	NucleicAcid		bind					TruB	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_929_s_102	11779468	(A) Superposition of the TSL  bound to TruB (colored as in     Figure 1) with  the corresponding residues from the structure of  tRNAPhe (in green).	bind
9352	1	3197	7	11	NULL	0	NULL	TSL	NucleicAcid		bind					TruB	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_929_s_102	11779468	(A) Superposition of the TSL  bound to TruB (colored as in     Figure 1) with  the corresponding residues from the structure of  tRNAPhe (in green).	bind
80035	1	3197	11	NULL	NULL	0	NULL	TSL	NucleicAcidSubstance		binds to 					 TruB	Protein				NULL		0	NULL	NULL	NULL	gw60_cell_107_7_929_s_102	11779468	(A) Superposition of the TSL  bound to TruB (colored as in     Figure 1) with  the corresponding residues from the structure of  tRNAPhe (in green).	bind
7811	1	3198	5	11	NULL	0	NULL	SWI/SNF	GP		bind					HO	GP			URS1	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4095_s_139	16705163	(A) SWI/SNF binding to  HO URS1 and URS2 is restored in a  gcn5 ash1 mutant.	bind
7821	2	3198	5	11	NULL	0	NULL	SWI/SNF	GP		bind					HO	GP			URS2	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4095_s_139	16705163	(A) SWI/SNF binding to  HO URS1 and URS2 is restored in a  gcn5 ash1 mutant.	bind
7823	3	3198	5	11	NULL	0	NULL	gcn5 ash1	GP	mutant	restore					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4095_s_139	16705163	(A) SWI/SNF binding to  HO URS1 and URS2 is restored in a  gcn5 ash1 mutant.	bind
7824	4	3198	5	11	NULL	0	NULL	gcn5 ash1	GP	mutant	restore					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4095_s_139	16705163	(A) SWI/SNF binding to  HO URS1 and URS2 is restored in a  gcn5 ash1 mutant.	bind
9353	1	3198	7	11	NULL	0	NULL	SWI/SNF	GP		bind					HO URS1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4095_s_139	16705163	(A) SWI/SNF binding to  HO URS1 and URS2 is restored in a  gcn5 ash1 mutant.	bind
9354	2	3198	7	11	NULL	0	NULL	SWI/SNF	GP		bind					HO URS2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4095_s_139	16705163	(A) SWI/SNF binding to  HO URS1 and URS2 is restored in a  gcn5 ash1 mutant.	bind
9355	3	3198	7	11	NULL	0	NULL	statement 1	Process		is restored in					gcn5 ash1 	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4095_s_139	16705163	(A) SWI/SNF binding to  HO URS1 and URS2 is restored in a  gcn5 ash1 mutant.	bind
9356	4	3198	7	11	NULL	0	NULL	statement 2	Process		is restored in					gcn5 ash1 	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4095_s_139	16705163	(A) SWI/SNF binding to  HO URS1 and URS2 is restored in a  gcn5 ash1 mutant.	bind
80036	1	3198	11	NULL	NULL	NULL	NULL	SWI/SNF	GeneOrProtein		binds to 					HO URS1	GeneOrProtein				NULL	gcn5 ash1 mutant	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4095_s_139	16705163	(A) SWI/SNF binding to  HO URS1 and URS2 is restored in a  gcn5 ash1 mutant.	bind
80037	2	3198	11	NULL	NULL	NULL	NULL	SWI/SNF	GeneOrProtein		binds to 					HO URS2	GeneOrProtein				NULL	gcn5 ash1 mutant.	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4095_s_139	16705163	(A) SWI/SNF binding to  HO URS1 and URS2 is restored in a  gcn5 ash1 mutant.	bind
7826	1	3201	5	11	NULL	0	NULL	eIF4G	GP		bind					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1678_2_67_s_251	15157733	(A) tail also affects the activity of maskin, a translational  inhibitor identified in  Xenopus oocytes, which competes with eIF4G binding to eIF4E.	bind
7828	2	3201	5	11	NULL	0	NULL	maskin	GP		bind					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1678_2_67_s_251	15157733	(A) tail also affects the activity of maskin, a translational  inhibitor identified in  Xenopus oocytes, which competes with eIF4G binding to eIF4E.	bind
7829	4	3201	5	11	NULL	0	NULL	statement 2	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1678_2_67_s_251	15157733	(A) tail also affects the activity of maskin, a translational  inhibitor identified in  Xenopus oocytes, which competes with eIF4G binding to eIF4E.	bind
7832	3	3201	5	11	NULL	0	NULL	maskin	GP		is a type of					translational inhibitor	GP				NULL	Xenopus oocytes	NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1678_2_67_s_251	15157733	(A) tail also affects the activity of maskin, a translational  inhibitor identified in  Xenopus oocytes, which competes with eIF4G binding to eIF4E.	bind
9489	1	3201	7	11	NULL	0	NULL	eIF4G	GP		bind					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1678_2_67_s_251	15157733	(A) tail also affects the activity of maskin, a translational  inhibitor identified in  Xenopus oocytes, which competes with eIF4G binding to eIF4E.	bind
9490	3	3201	7	11	NULL	0	NULL	Maskin	GP		bind					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1678_2_67_s_251	15157733	(A) tail also affects the activity of maskin, a translational  inhibitor identified in  Xenopus oocytes, which competes with eIF4G binding to eIF4E.	bind
9491	4	3201	7	11	NULL	0	NULL	statement 3	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1678_2_67_s_251	15157733	(A) tail also affects the activity of maskin, a translational  inhibitor identified in  Xenopus oocytes, which competes with eIF4G binding to eIF4E.	bind
12362	2	3201	7	11	NULL	0	NULL	Maskin	GP		is a type of					translational inhibitor	GP				NULL	Xenopus oocytes	NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1678_2_67_s_251	15157733	(A) tail also affects the activity of maskin, a translational  inhibitor identified in  Xenopus oocytes, which competes with eIF4G binding to eIF4E.	bind
80038	1	3201	11	NULL	NULL	0	NULL	maskin	Protein		is a type of 					translational inhibitor	Protein				NULL	Xenopus oocytes	0	NULL	NULL	NULL	gw70_biochimbiophysacta_1678_2_67_s_251	15157733	(A) tail also affects the activity of maskin, a translational  inhibitor identified in  Xenopus oocytes, which competes with eIF4G binding to eIF4E.	bind
80039	2	3201	11	NULL	NULL	NULL	NULL	eIF4G	GeneOrProtein		binds to 					eIF4E	GeneOrProtein				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1678_2_67_s_251	15157733	(A) tail also affects the activity of maskin, a translational  inhibitor identified in  Xenopus oocytes, which competes with eIF4G binding to eIF4E.	bind
80040	3	3201	11	NULL	NULL	NULL	NULL	maskin	GeneOrProtein		binds to 					eIF4E	GeneOrProtein				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1678_2_67_s_251	15157733	(A) tail also affects the activity of maskin, a translational  inhibitor identified in  Xenopus oocytes, which competes with eIF4G binding to eIF4E.	bind
80041	4	3201	11	NULL	NULL	0	NULL	statement 2	Process		competes with					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1678_2_67_s_251	15157733	(A) tail also affects the activity of maskin, a translational  inhibitor identified in  Xenopus oocytes, which competes with eIF4G binding to eIF4E.	bind
7838	1	3202	5	11	NULL	0	NULL	eIF4A	GP		bind						NucleicAcid			5' UTR	NULL		NULL	NULL	NULL	NULL	gw60_nature_392_6675_520_s_79	9548260	(A) tail and eIF4A bound to the 5' UTR ( Fig. 4a).	bind
9492	1	3202	7	11	NULL	0	NULL	eIF4A	GP		bind						NucleicAcid			5' UTR	NULL		NULL	NULL	NULL	NULL	gw60_nature_392_6675_520_s_79	9548260	(A) tail and eIF4A bound to the 5' UTR ( Fig. 4a).	bind
80042	1	3202	11	NULL	NULL	0	NULL	(A) tail	NucleicAcidSubstance		binds to 					5' UTR	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_nature_392_6675_520_s_79	9548260	(A) tail and eIF4A bound to the 5' UTR ( Fig. 4a).	bind
80043	2	3202	11	NULL	NULL	NULL	NULL	eIF4A	GeneOrProtein		binds to 					5' UTR	NucleicAcidSubstance				NULL		NULL	NULL	NULL	NULL	gw60_nature_392_6675_520_s_79	9548260	(A) tail and eIF4A bound to the 5' UTR ( Fig. 4a).	bind
7846	1	3203	5	11	NULL	0	NULL	Unr protein	GP		bind					mCRD	NucleicAcid			purine stretches	NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_29_s_290	11051545	(A) tail and the Unr protein binds to the purine stretches in  the mCRD.	bind
9493	1	3203	7	11	NULL	0	NULL	Unr protein	GP		bind					mCRD	NucleicAcid			purine stretches	NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_29_s_290	11051545	(A) tail and the Unr protein binds to the purine stretches in  the mCRD.	bind
80044	1	3203	11	NULL	NULL	0	NULL	(A) tail 	NucleicAcidSubstance		binds to 					mCRD	GeneOrProtein			 purine stretches	NULL		0	NULL	NULL	NULL	gw60_cell_103_1_29_s_290	11051545	(A) tail and the Unr protein binds to the purine stretches in  the mCRD.	bind
80045	2	3203	11	NULL	NULL	0	NULL	Unr protein	Protein		binds to 					mCRD	GeneOrProtein			purine stretches	NULL		0	NULL	NULL	NULL	gw60_cell_103_1_29_s_290	11051545	(A) tail and the Unr protein binds to the purine stretches in  the mCRD.	bind
7879	1	3204	5	11	NULL	0	NULL	eIF4E	GP		bind					eIF4G	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_21_4068_s_19	11058101	(A) tail are recognised, respectively, by the eukaryotic initiation factor (eIF) 4F holoenzyme complex [consisting of the cap-binding protein (eIF4E) and an ATP-dependent RNA helicase (eIF4A) bound to a central scaffold molecule (eIF4G)] (for reviews see  3, 9) and by the poly	bind
7880	2	3204	5	11	NULL	0	NULL	eIF4A	GP		bind					eIF4G	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_21_4068_s_19	11058101	(A) tail are recognised, respectively, by the eukaryotic initiation factor (eIF) 4F holoenzyme complex [consisting of the cap-binding protein (eIF4E) and an ATP-dependent RNA helicase (eIF4A) bound to a central scaffold molecule (eIF4G)] (for reviews see  3, 9) and by the poly	bind
7881	3	3204	5	11	NULL	0	NULL	(eIF) 4F holoenzyme complex	GP		consists of					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_21_4068_s_19	11058101	(A) tail are recognised, respectively, by the eukaryotic initiation factor (eIF) 4F holoenzyme complex [consisting of the cap-binding protein (eIF4E) and an ATP-dependent RNA helicase (eIF4A) bound to a central scaffold molecule (eIF4G)] (for reviews see  3, 9) and by the poly	bind
9494	1	3204	7	11	NULL	0	NULL	eIF4E	GP		bind					eIF4G	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_21_4068_s_19	11058101	(A) tail are recognised, respectively, by the eukaryotic initiation factor (eIF) 4F holoenzyme complex [consisting of the cap-binding protein (eIF4E) and an ATP-dependent RNA helicase (eIF4A) bound to a central scaffold molecule (eIF4G)] (for reviews see  3, 9) and by the poly	bind
9495	2	3204	7	11	NULL	0	NULL	eIF4A	GP		bind					eIF4G	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_21_4068_s_19	11058101	(A) tail are recognised, respectively, by the eukaryotic initiation factor (eIF) 4F holoenzyme complex [consisting of the cap-binding protein (eIF4E) and an ATP-dependent RNA helicase (eIF4A) bound to a central scaffold molecule (eIF4G)] (for reviews see  3, 9) and by the poly	bind
9496	3	3204	7	11	NULL	0	NULL	eukaryotic initiation factor 4F holoenzyme complex	GP		consist of					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_21_4068_s_19	11058101	(A) tail are recognised, respectively, by the eukaryotic initiation factor (eIF) 4F holoenzyme complex [consisting of the cap-binding protein (eIF4E) and an ATP-dependent RNA helicase (eIF4A) bound to a central scaffold molecule (eIF4G)] (for reviews see  3, 9) and by the poly	bind
9497	4	3204	7	11	NULL	0	NULL	eukaryotic initiation factor 4F holoenzyme complex	GP		consist of					eIF4A	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_21_4068_s_19	11058101	(A) tail are recognised, respectively, by the eukaryotic initiation factor (eIF) 4F holoenzyme complex [consisting of the cap-binding protein (eIF4E) and an ATP-dependent RNA helicase (eIF4A) bound to a central scaffold molecule (eIF4G)] (for reviews see  3, 9) and by the poly	bind
9498	5	3204	7	11	NULL	0	NULL	 eukaryotic initiation factor 	GP		is					eIF	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_21_4068_s_19	11058101	(A) tail are recognised, respectively, by the eukaryotic initiation factor (eIF) 4F holoenzyme complex [consisting of the cap-binding protein (eIF4E) and an ATP-dependent RNA helicase (eIF4A) bound to a central scaffold molecule (eIF4G)] (for reviews see  3, 9) and by the poly	bind
9499	6	3204	7	11	NULL	0	NULL	eIF4E	GP		is a type of					cap-binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_21_4068_s_19	11058101	(A) tail are recognised, respectively, by the eukaryotic initiation factor (eIF) 4F holoenzyme complex [consisting of the cap-binding protein (eIF4E) and an ATP-dependent RNA helicase (eIF4A) bound to a central scaffold molecule (eIF4G)] (for reviews see  3, 9) and by the poly	bind
9500	7	3204	7	11	NULL	0	NULL	eIF4A	GP		is a type of					ATP-dependent RNA helicase 	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_21_4068_s_19	11058101	(A) tail are recognised, respectively, by the eukaryotic initiation factor (eIF) 4F holoenzyme complex [consisting of the cap-binding protein (eIF4E) and an ATP-dependent RNA helicase (eIF4A) bound to a central scaffold molecule (eIF4G)] (for reviews see  3, 9) and by the poly	bind
9501	8	3204	7	11	NULL	0	NULL	eIF4G	GP		is a type of					central scaffold molecule	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_21_4068_s_19	11058101	(A) tail are recognised, respectively, by the eukaryotic initiation factor (eIF) 4F holoenzyme complex [consisting of the cap-binding protein (eIF4E) and an ATP-dependent RNA helicase (eIF4A) bound to a central scaffold molecule (eIF4G)] (for reviews see  3, 9) and by the poly	bind
80046	1	3204	11	NULL	NULL	NULL	NULL	eukaryotic initiation factor 4F	Protein		is a part of					holoenzyme complex	Protein				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_21_4068_s_19	11058101	(A) tail are recognised, respectively, by the eukaryotic initiation factor (eIF) 4F holoenzyme complex [consisting of the cap-binding protein (eIF4E) and an ATP-dependent RNA helicase (eIF4A) bound to a central scaffold molecule (eIF4G)] (for reviews see  3, 9) and by the poly	bind
80047	2	3204	11	NULL	NULL	NULL	NULL	holoenzyme complex	Protein		consisting of 					cap-binding protein	Protein				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_21_4068_s_19	11058101	(A) tail are recognised, respectively, by the eukaryotic initiation factor (eIF) 4F holoenzyme complex [consisting of the cap-binding protein (eIF4E) and an ATP-dependent RNA helicase (eIF4A) bound to a central scaffold molecule (eIF4G)] (for reviews see  3, 9) and by the poly	bind
80048	3	3204	11	NULL	NULL	0	NULL	eIF4E	Protein		is a type of 					cap-binding protein	Protein				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_21_4068_s_19	11058101	(A) tail are recognised, respectively, by the eukaryotic initiation factor (eIF) 4F holoenzyme complex [consisting of the cap-binding protein (eIF4E) and an ATP-dependent RNA helicase (eIF4A) bound to a central scaffold molecule (eIF4G)] (for reviews see  3, 9) and by the poly	bind
80049	4	3204	11	NULL	NULL	NULL	NULL	holoenzyme complex	Protein		consisting of 					RNA helicase 	Protein	ATP-dependent			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_21_4068_s_19	11058101	(A) tail are recognised, respectively, by the eukaryotic initiation factor (eIF) 4F holoenzyme complex [consisting of the cap-binding protein (eIF4E) and an ATP-dependent RNA helicase (eIF4A) bound to a central scaffold molecule (eIF4G)] (for reviews see  3, 9) and by the poly	bind
80050	5	3204	11	NULL	NULL	0	NULL	eIF4A	Protein		is a type of 					RNA helicase 	Protein	ATP-dependent			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_21_4068_s_19	11058101	(A) tail are recognised, respectively, by the eukaryotic initiation factor (eIF) 4F holoenzyme complex [consisting of the cap-binding protein (eIF4E) and an ATP-dependent RNA helicase (eIF4A) bound to a central scaffold molecule (eIF4G)] (for reviews see  3, 9) and by the poly	bind
80051	6	3204	11	NULL	NULL	0	NULL	holoenzyme complex	Protein		consisting of 					eIF4G	Protein				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_21_4068_s_19	11058101	(A) tail are recognised, respectively, by the eukaryotic initiation factor (eIF) 4F holoenzyme complex [consisting of the cap-binding protein (eIF4E) and an ATP-dependent RNA helicase (eIF4A) bound to a central scaffold molecule (eIF4G)] (for reviews see  3, 9) and by the poly	bind
80052	7	3204	11	NULL	NULL	0	NULL	eIF4E	Protein		binds to 					eIF4G	Protein				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_21_4068_s_19	11058101	(A) tail are recognised, respectively, by the eukaryotic initiation factor (eIF) 4F holoenzyme complex [consisting of the cap-binding protein (eIF4E) and an ATP-dependent RNA helicase (eIF4A) bound to a central scaffold molecule (eIF4G)] (for reviews see  3, 9) and by the poly	bind
80053	8	3204	11	NULL	NULL	0	NULL	eIF4A	Protein		binds to 					eIF4G	Protein				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_21_4068_s_19	11058101	(A) tail are recognised, respectively, by the eukaryotic initiation factor (eIF) 4F holoenzyme complex [consisting of the cap-binding protein (eIF4E) and an ATP-dependent RNA helicase (eIF4A) bound to a central scaffold molecule (eIF4G)] (for reviews see  3, 9) and by the poly	bind
7884	1	3205	5	11	NULL	0	NULL	NSP3	GP	viral 	interact with					eIF4GI	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0760-0779_j-virol_80_18_16940515_s_8	16940515	(A) tail but have instead  a consensus sequence at their 3' ends that is bound by the viral nonstructural  protein NSP3, which also interacts with eIF4GI, using the same region  employed by PABP.	bind
9502	1	3205	7	11	NULL	0	NULL	NSP3	GP	viral 	bind					eIF4GI	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0760-0779_j-virol_80_18_16940515_s_8	16940515	(A) tail but have instead  a consensus sequence at their 3' ends that is bound by the viral nonstructural  protein NSP3, which also interacts with eIF4GI, using the same region  employed by PABP.	bind
80054	1	3205	11	NULL	NULL	0	NULL	(A) tail	NucleicAcidSubstance		has					consensus sequence	NucleicAcidSubstance			 3' ends	NULL		0	NULL	NULL	NULL	abs-batch0760-0779_j-virol_80_18_16940515_s_8	16940515	(A) tail but have instead  a consensus sequence at their 3' ends that is bound by the viral nonstructural  protein NSP3, which also interacts with eIF4GI, using the same region  employed by PABP.	bind
80055	2	3205	11	NULL	NULL	0	NULL	statement 1	NucleicAcidSubstance		binds to 					NSP3	Protein				NULL		0	NULL	NULL	NULL	abs-batch0760-0779_j-virol_80_18_16940515_s_8	16940515	(A) tail but have instead  a consensus sequence at their 3' ends that is bound by the viral nonstructural  protein NSP3, which also interacts with eIF4GI, using the same region  employed by PABP.	bind
80056	3	3205	11	NULL	NULL	0	NULL	NSP3	Protein		is a type of 					nonstructural protein	Protein	viral 			NULL		0	NULL	NULL	NULL	abs-batch0760-0779_j-virol_80_18_16940515_s_8	16940515	(A) tail but have instead  a consensus sequence at their 3' ends that is bound by the viral nonstructural  protein NSP3, which also interacts with eIF4GI, using the same region  employed by PABP.	bind
80057	4	3205	11	NULL	NULL	0	NULL	NSP3	Protein		interact with					eIF4GI	Protein				NULL		0	NULL	NULL	NULL	abs-batch0760-0779_j-virol_80_18_16940515_s_8	16940515	(A) tail but have instead  a consensus sequence at their 3' ends that is bound by the viral nonstructural  protein NSP3, which also interacts with eIF4GI, using the same region  employed by PABP.	bind
8709	1	3206	5	11	NULL	0	NULL	Maskin	GP		is displaced from					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_47_16961_s_239	16287976	(A) tail elongation leading to PABP-binding, recruitment of eIF4G, displacement of Maskin from eIF4E, and activation of translation ( ).	bind
9504	1	3206	7	11	NULL	0	NULL	Maskin	GP		displaced from					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_47_16961_s_239	16287976	(A) tail elongation leading to PABP-binding, recruitment of eIF4G, displacement of Maskin from eIF4E, and activation of translation ( ).	bind
80058	1	3206	11	NULL	NULL	0	NULL	elongation	MolecularProcess	(A) tail	binds to 					PABP	Protein				NULL		0	NULL	NULL	NULL	gw70_pnas_102_47_16961_s_239	16287976	(A) tail elongation leading to PABP-binding, recruitment of eIF4G, displacement of Maskin from eIF4E, and activation of translation ( ).	bind
80059	2	3206	11	NULL	NULL	0	NULL	elongation	MolecularProcess	(A) tail	recruit					eIF4G	Protein				NULL		0	NULL	NULL	NULL	gw70_pnas_102_47_16961_s_239	16287976	(A) tail elongation leading to PABP-binding, recruitment of eIF4G, displacement of Maskin from eIF4E, and activation of translation ( ).	bind
80060	3	3206	11	NULL	NULL	0	NULL	Maskin	Protein		binds to 					eIF4E	Protein				NULL		0	NULL	NULL	NULL	gw70_pnas_102_47_16961_s_239	16287976	(A) tail elongation leading to PABP-binding, recruitment of eIF4G, displacement of Maskin from eIF4E, and activation of translation ( ).	bind
80061	4	3206	11	NULL	NULL	NULL	NULL	elongation	MolecularProcess	(A) tail	displaces					Maskin	Protein	from eIF4E			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_47_16961_s_239	16287976	(A) tail elongation leading to PABP-binding, recruitment of eIF4G, displacement of Maskin from eIF4E, and activation of translation ( ).	bind
80062	5	3206	11	NULL	NULL	NULL	NULL	elongation	MolecularProcess	(A) tail	activates					translation	MolecularProcess				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_47_16961_s_239	16287976	(A) tail elongation leading to PABP-binding, recruitment of eIF4G, displacement of Maskin from eIF4E, and activation of translation ( ).	bind
80063	1	3208	11	NULL	NULL	0	NULL	CPSF	Protein		binds to 					(A) tail	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1315_s_138	15937220	(A) tail length control is dependent upon the binding of both CPSF and PABPN1 (Wahle 1995 ), the extended poly	bind
80064	2	3208	11	NULL	NULL	0	NULL	PABPN1	Protein		binds to 					(A) tail	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1315_s_138	15937220	(A) tail length control is dependent upon the binding of both CPSF and PABPN1 (Wahle 1995 ), the extended poly	bind
80065	3	3208	11	NULL	NULL	0	NULL	statement 1	Process		controls					length	Measurement	(A) tail 			NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1315_s_138	15937220	(A) tail length control is dependent upon the binding of both CPSF and PABPN1 (Wahle 1995 ), the extended poly	bind
80066	4	3208	11	NULL	NULL	0	NULL	statement 2	Process		controls					length	Measurement	(A) tail 			NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1315_s_138	15937220	(A) tail length control is dependent upon the binding of both CPSF and PABPN1 (Wahle 1995 ), the extended poly	bind
80067	5	3208	11	NULL	NULL	0	NULL	statement 3	Process		occurs along with					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_11_1315_s_138	15937220	(A) tail length control is dependent upon the binding of both CPSF and PABPN1 (Wahle 1995 ), the extended poly	bind
7889	1	3209	5	11	NULL	0	NULL	eIF4G	GP		bind					PABP/poly	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_19_2510_s_273	9334316	(A) tail or the binding of eIF4G to the PABP/poly	bind
9505	1	3209	7	11	NULL	0	NULL	eIF4G	GP		bind					PABP/poly	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_19_2510_s_273	9334316	(A) tail or the binding of eIF4G to the PABP/poly	bind
7890	1	3210	5	11	NULL	0	NULL	initiation factor	GP		bind					m7G cap	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_1_104_s_186	15630022	(A) tail stimulates initiation factor binding to the m7G cap.	bind
9506	1	3210	7	11	NULL	0	NULL	initiation factor	GP		bind					m7G cap	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_1_104_s_186	15630022	(A) tail stimulates initiation factor binding to the m7G cap.	bind
80068	1	3210	11	NULL	NULL	0	NULL	initiation factor	Protein		binds to 					m7G cap	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_1_104_s_186	15630022	(A) tail stimulates initiation factor binding to the m7G cap.	bind
80069	2	3210	11	NULL	NULL	0	NULL	(A) tail	NucleicAcidSubstance		stimulates					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_1_104_s_186	15630022	(A) tail stimulates initiation factor binding to the m7G cap.	bind
7892	1	3211	5	11	NULL	0	NULL	PABPN1	GP		bind					NS1 protein	GP	influenza virus			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1678_2_67_s_481	15157733	(A) tail synthesis has been confirmed in vivo: PABPN1  is bound and inactivated by the influenza virus protein NS1, and mRNAs containing  very short oligo	bind
7893	2	3211	5	11	NULL	0	NULL	NS1 protein	GP	influenza virus	inactivate					PABPN1	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1678_2_67_s_481	15157733	(A) tail synthesis has been confirmed in vivo: PABPN1  is bound and inactivated by the influenza virus protein NS1, and mRNAs containing  very short oligo	bind
9508	1	3211	7	11	NULL	0	NULL	PABPN1	GP		binds					NS1 protein	GP	influenza virus 			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1678_2_67_s_481	15157733	(A) tail synthesis has been confirmed in vivo: PABPN1  is bound and inactivated by the influenza virus protein NS1, and mRNAs containing  very short oligo	bind
9509	2	3211	7	11	NULL	0	NULL	NS1 protein	GP	influenza virus 	inactivate					PABPN1	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1678_2_67_s_481	15157733	(A) tail synthesis has been confirmed in vivo: PABPN1  is bound and inactivated by the influenza virus protein NS1, and mRNAs containing  very short oligo	bind
80070	1	3211	11	NULL	NULL	0	NULL	NS1 protein	Protein	influenza virus	binds to 					PABPN1	Protein				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1678_2_67_s_481	15157733	(A) tail synthesis has been confirmed in vivo: PABPN1  is bound and inactivated by the influenza virus protein NS1, and mRNAs containing  very short oligo	bind
80071	2	3211	11	NULL	NULL	0	NULL	NS1 protein	Protein	influenza virus	inactivates					PABPN1	Protein				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1678_2_67_s_481	15157733	(A) tail synthesis has been confirmed in vivo: PABPN1  is bound and inactivated by the influenza virus protein NS1, and mRNAs containing  very short oligo	bind
80072	3	3211	11	NULL	NULL	0	NULL	statement 1	Process		occurs along with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1678_2_67_s_481	15157733	(A) tail synthesis has been confirmed in vivo: PABPN1  is bound and inactivated by the influenza virus protein NS1, and mRNAs containing  very short oligo	bind
7896	1	3212	5	11	NULL	0	NULL	GST-RNG105	GP		bind					brain RNA	NucleicAcid	rat 			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jneurosci_25_17_4420_s_273	15858068	(A) tails in the  in vitro binding assay showed that the binding of GST-RNG105 to rat brain RNAs was not significantly altered in the presence or absence of poly(dT), suggesting that poly	bind
9510	1	3212	7	11	NULL	0	NULL	GST-RNG105	GP		binds					brain RNA	NucleicAcid	rat			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jneurosci_25_17_4420_s_273	15858068	(A) tails in the  in vitro binding assay showed that the binding of GST-RNG105 to rat brain RNAs was not significantly altered in the presence or absence of poly(dT), suggesting that poly	bind
80073	1	3212	11	NULL	NULL	0	NULL	GST-RNG105	Protein		binds to 					RNAs	NucleicAcidSubstance	 rat brain 			NULL		0	NULL	NULL	NULL	gw70_jneurosci_25_17_4420_s_273	15858068	(A) tails in the  in vitro binding assay showed that the binding of GST-RNG105 to rat brain RNAs was not significantly altered in the presence or absence of poly(dT), suggesting that poly	bind
80074	2	3212	11	NULL	NULL	0	NULL	statement 1	Process		is independent of					poly(dT)	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_jneurosci_25_17_4420_s_273	15858068	(A) tails in the  in vitro binding assay showed that the binding of GST-RNG105 to rat brain RNAs was not significantly altered in the presence or absence of poly(dT), suggesting that poly	bind
7897	1	3213	5	11	NULL	0	NULL	PABPs	GP		bind					DAZL	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_14_2656_s_314	16001084	(A) tails may  benefit the most from the binding of PABPs to DAZL, as seen in  Figures 3 and  7.	bind
9511	1	3213	7	11	NULL	0	NULL	PABPs	GP		bind					DAZL	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_14_2656_s_314	16001084	(A) tails may  benefit the most from the binding of PABPs to DAZL, as seen in  Figures 3 and  7.	bind
80075	1	3213	11	NULL	NULL	0	NULL	PABPs	Protein		binds to 					DAZL	Protein				NULL		0	NULL	NULL	NULL	gw70_embo_24_14_2656_s_314	16001084	(A) tails may  benefit the most from the binding of PABPs to DAZL, as seen in  Figures 3 and  7.	bind
7898	1	3215	5	11	NULL	0	NULL	Tbx5	GP		bind					GST-LIM2/3	GP				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_273_1_106_s_131	15302601	(A) Tbx5 binds to GST-LIM2/3.	bind
9512	1	3215	7	11	NULL	0	NULL	Tbx5	GP		binds					GST-LIM2/3	GP				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_273_1_106_s_131	15302601	(A) Tbx5 binds to GST-LIM2/3.	bind
80076	1	3215	11	NULL	NULL	0	NULL	Tbx5	Protein		binds to 					GST-LIM2/3	Protein				NULL		0	NULL	NULL	NULL	gw70_devbiol_273_1_106_s_131	15302601	(A) Tbx5 binds to GST-LIM2/3.	bind
7899	1	3216	5	11	NULL	0	NULL	TCR-CD3	GP		bind					Nck	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_109_7_901_s_129	12110186	(A) TCR-CD3 binding to Nck is independent of tyrosine phosphorylation.	bind
7900	2	3216	5	11	NULL	0	NULL	statement 1	Process		is independent of							phosphorylation	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_cell_109_7_901_s_129	12110186	(A) TCR-CD3 binding to Nck is independent of tyrosine phosphorylation.	bind
9513	1	3216	7	11	NULL	0	NULL	TCR-CD3	GP		binds					Nck	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_109_7_901_s_129	12110186	(A) TCR-CD3 binding to Nck is independent of tyrosine phosphorylation.	bind
9514	2	3216	7	11	NULL	0	NULL	statement 1	Process		is independent of					 		phosphorylation 	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_cell_109_7_901_s_129	12110186	(A) TCR-CD3 binding to Nck is independent of tyrosine phosphorylation.	bind
80077	1	3216	11	NULL	NULL	0	NULL	TCR-CD3	Protein		binds to 					Nck	Protein				NULL		0	NULL	NULL	NULL	gw60_cell_109_7_901_s_129	12110186	(A) TCR-CD3 binding to Nck is independent of tyrosine phosphorylation.	bind
80078	2	3216	11	NULL	NULL	0	NULL	statement 1	Process		is independent of					phosphorylation	MolecularProcess	tyrosine			NULL		0	NULL	NULL	NULL	gw60_cell_109_7_901_s_129	12110186	(A) TCR-CD3 binding to Nck is independent of tyrosine phosphorylation.	bind
7901	1	3218	5	11	NULL	0	NULL	Tet(O)	GP		bind					fMet-tRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_5_1037_s_84	11389850	(a) Tet(O) bound to fMet-tRNA.	bind
9515	1	3218	7	11	NULL	0	NULL	Tet(O)	GP		bind					fMet-tRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_5_1037_s_84	11389850	(a) Tet(O) bound to fMet-tRNA.	bind
80079	1	3218	11	NULL	NULL	0	NULL	Tet(O)	Protein		binds to 					fMet-tRNA	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcell_7_5_1037_s_84	11389850	(a) Tet(O) bound to fMet-tRNA.	bind
7903	1	3219	5	11	NULL	0	NULL	p300 fragments	GP		end at			carboxy-terminal 					amino acid 2414		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_71	10330164	(A) TFIIB binds to p300 carboxy-terminal fragments ending at amino acids 2414, 1906, and 1710.	bind
7904	2	3219	5	11	NULL	0	NULL	p300 fragments	GP		end at			carboxy-terminal					amino acid 1906		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_71	10330164	(A) TFIIB binds to p300 carboxy-terminal fragments ending at amino acids 2414, 1906, and 1710.	bind
7905	3	3219	5	11	NULL	0	NULL	p300 fragments	GP		end at			carboxy-terminal					amino acid 1710		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_71	10330164	(A) TFIIB binds to p300 carboxy-terminal fragments ending at amino acids 2414, 1906, and 1710.	bind
7906	4	3219	5	11	NULL	0	NULL	TFIIB	GP		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_71	10330164	(A) TFIIB binds to p300 carboxy-terminal fragments ending at amino acids 2414, 1906, and 1710.	bind
7907	5	3219	5	11	NULL	0	NULL	TFIIB	GP		bind					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_71	10330164	(A) TFIIB binds to p300 carboxy-terminal fragments ending at amino acids 2414, 1906, and 1710.	bind
7908	6	3219	5	11	NULL	0	NULL	TFIIB	GP		bind					statement 3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_71	10330164	(A) TFIIB binds to p300 carboxy-terminal fragments ending at amino acids 2414, 1906, and 1710.	bind
9516	1	3219	7	11	NULL	0	NULL	p300 fragments	GP		end at			carboxy-terminal					amino acids 2414		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_71	10330164	(A) TFIIB binds to p300 carboxy-terminal fragments ending at amino acids 2414, 1906, and 1710.	bind
12367	2	3219	7	11	NULL	0	NULL	p300 fragments	GP		end at			carboxy-terminal					amino acids 1906		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_71	10330164	(A) TFIIB binds to p300 carboxy-terminal fragments ending at amino acids 2414, 1906, and 1710.	bind
12369	3	3219	7	11	NULL	0	NULL	p300 fragments	GP		end at			carboxy-terminal					amino acids 1710		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_71	10330164	(A) TFIIB binds to p300 carboxy-terminal fragments ending at amino acids 2414, 1906, and 1710.	bind
12371	4	3219	7	11	NULL	0	NULL	TFIIB	GP		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_71	10330164	(A) TFIIB binds to p300 carboxy-terminal fragments ending at amino acids 2414, 1906, and 1710.	bind
12373	5	3219	7	11	NULL	0	NULL	TFIIB	GP		bind					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_71	10330164	(A) TFIIB binds to p300 carboxy-terminal fragments ending at amino acids 2414, 1906, and 1710.	bind
12374	6	3219	7	11	NULL	0	NULL	TFIIB	GP		bind					statement 3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_71	10330164	(A) TFIIB binds to p300 carboxy-terminal fragments ending at amino acids 2414, 1906, and 1710.	bind
80111	1	3219	11	NULL	NULL	0	NULL	TFIIB	Protein		binds to 					p300	Protein	carboxy-terminal	amino acids 2414, 1906, and 1710		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_71	10330164	(A) TFIIB binds to p300 carboxy-terminal fragments ending at amino acids 2414, 1906, and 1710.	bind
7910	1	3221	5	11	NULL	0	NULL	Flo8	GP		bind									UAS1-2	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_214	15485921	(A) The  ste12delta and  tec1delta mutations eliminate Flo8 and Mss11 binding to UAS1-2.	bind
7911	2	3221	5	11	NULL	0	NULL	Mss11	GP		bind									UAS1-2	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_214	15485921	(A) The  ste12delta and  tec1delta mutations eliminate Flo8 and Mss11 binding to UAS1-2.	bind
7914	3	3221	5	11	NULL	0	NULL	 ste12delta	GP	mutant	eliminate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_214	15485921	(A) The  ste12delta and  tec1delta mutations eliminate Flo8 and Mss11 binding to UAS1-2.	bind
7915	4	3221	5	11	NULL	0	NULL	ste12delta	GP	mutant	eliminate					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_214	15485921	(A) The  ste12delta and  tec1delta mutations eliminate Flo8 and Mss11 binding to UAS1-2.	bind
7916	5	3221	5	11	NULL	0	NULL	tec1delta	GP	mutant	eliminate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_214	15485921	(A) The  ste12delta and  tec1delta mutations eliminate Flo8 and Mss11 binding to UAS1-2.	bind
7917	6	3221	5	11	NULL	0	NULL	 tec1delta	GP	mutant	eliminate					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_214	15485921	(A) The  ste12delta and  tec1delta mutations eliminate Flo8 and Mss11 binding to UAS1-2.	bind
9517	1	3221	7	11	NULL	0	NULL	Flo8	GP		bind									UAS1-2	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_214	15485921	(A) The  ste12delta and  tec1delta mutations eliminate Flo8 and Mss11 binding to UAS1-2.	bind
9518	2	3221	7	11	NULL	0	NULL	Mss11	GP		bind									UAS1-2	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_214	15485921	(A) The  ste12delta and  tec1delta mutations eliminate Flo8 and Mss11 binding to UAS1-2.	bind
9519	3	3221	7	11	NULL	0	NULL	ste12delta	GP	mutant	eliminate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_214	15485921	(A) The  ste12delta and  tec1delta mutations eliminate Flo8 and Mss11 binding to UAS1-2.	bind
9520	4	3221	7	11	NULL	0	NULL	ste12delta	GP	mutant	eliminate					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_214	15485921	(A) The  ste12delta and  tec1delta mutations eliminate Flo8 and Mss11 binding to UAS1-2.	bind
9521	5	3221	7	11	NULL	0	NULL	 tec1delta	GP	mutant	eliminate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_214	15485921	(A) The  ste12delta and  tec1delta mutations eliminate Flo8 and Mss11 binding to UAS1-2.	bind
9522	6	3221	7	11	NULL	0	NULL	 tec1delta	GP	mutant	eliminate					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_214	15485921	(A) The  ste12delta and  tec1delta mutations eliminate Flo8 and Mss11 binding to UAS1-2.	bind
80112	1	3221	11	NULL	NULL	0	NULL	Mss11	Protein		binds to 					UAS1-2	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_214	15485921	(A) The  ste12delta and  tec1delta mutations eliminate Flo8 and Mss11 binding to UAS1-2.	bind
80113	2	3221	11	NULL	NULL	0	NULL	Flo8	Protein		binds to 					UAS1-2	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_214	15485921	(A) The  ste12delta and  tec1delta mutations eliminate Flo8 and Mss11 binding to UAS1-2.	bind
80114	3	3221	11	NULL	NULL	NULL	NULL	ste12delta	GeneOrProtein	mutation of	eliminate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_214	15485921	(A) The  ste12delta and  tec1delta mutations eliminate Flo8 and Mss11 binding to UAS1-2.	bind
80115	4	3221	11	NULL	NULL	0	NULL	ste12delta	GeneOrProtein	mutation of	eliminate					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_214	15485921	(A) The  ste12delta and  tec1delta mutations eliminate Flo8 and Mss11 binding to UAS1-2.	bind
80116	5	3221	11	NULL	NULL	0	NULL	tec1delta	GeneOrProtein	mutation of	eliminate					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_214	15485921	(A) The  ste12delta and  tec1delta mutations eliminate Flo8 and Mss11 binding to UAS1-2.	bind
80117	6	3221	11	NULL	NULL	0	NULL	tec1delta	GeneOrProtein	mutation of	eliminate					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_214	15485921	(A) The  ste12delta and  tec1delta mutations eliminate Flo8 and Mss11 binding to UAS1-2.	bind
7918	1	3222	5	11	NULL	0	NULL	ste50delta 	GP		effect					cell cycle arrest	Process	pheromone-induced 			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_7_2425_s_189	10397774	(A) The  ste50delta and the deletion of Ste50p binding domain of Ste11p had the same effect on the pheromone-induced cell cycle arrest.	bind
7919	2	3222	5	11	NULL	0	NULL				deleted from			Ste50p binding domain		Ste11p	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_7_2425_s_189	10397774	(A) The  ste50delta and the deletion of Ste50p binding domain of Ste11p had the same effect on the pheromone-induced cell cycle arrest.	bind
7920	3	3222	5	11	NULL	0	NULL	statement 2	Process		effect					cell cycle arrest	Process	pheromone-induced			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_7_2425_s_189	10397774	(A) The  ste50delta and the deletion of Ste50p binding domain of Ste11p had the same effect on the pheromone-induced cell cycle arrest.	bind
7921	4	3222	5	11	NULL	0	NULL	statement 1	Process		same effect as					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_7_2425_s_189	10397774	(A) The  ste50delta and the deletion of Ste50p binding domain of Ste11p had the same effect on the pheromone-induced cell cycle arrest.	bind
9523	1	3222	7	11	NULL	0	NULL	pheromone	Chemical		induce					cell cycle arrest	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_7_2425_s_189	10397774	(A) The  ste50delta and the deletion of Ste50p binding domain of Ste11p had the same effect on the pheromone-induced cell cycle arrest.	bind
9524	2	3222	7	11	NULL	0	NULL	ste50delta	GP		effect					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_7_2425_s_189	10397774	(A) The  ste50delta and the deletion of Ste50p binding domain of Ste11p had the same effect on the pheromone-induced cell cycle arrest.	bind
9525	3	3222	7	11	NULL	0	NULL	Ste11p	GP	deletion of	effect			Ste50p binding domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_7_2425_s_189	10397774	(A) The  ste50delta and the deletion of Ste50p binding domain of Ste11p had the same effect on the pheromone-induced cell cycle arrest.	bind
12377	4	3222	7	11	NULL	0	NULL	statement 2	Process		same effect as					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_7_2425_s_189	10397774	(A) The  ste50delta and the deletion of Ste50p binding domain of Ste11p had the same effect on the pheromone-induced cell cycle arrest.	bind
80118	1	3222	11	NULL	NULL	0	NULL	pheromone	Chemical		induced					cell cycle arrest	MolecularProcess				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_10_7_2425_s_189	10397774	(A) The  ste50delta and the deletion of Ste50p binding domain of Ste11p had the same effect on the pheromone-induced cell cycle arrest.	bind
80119	2	3222	11	NULL	NULL	0	NULL	Ste11p	GeneOrProtein		has binding domain for					Ste50p	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_10_7_2425_s_189	10397774	(A) The  ste50delta and the deletion of Ste50p binding domain of Ste11p had the same effect on the pheromone-induced cell cycle arrest.	bind
7922	1	3223	5	11	NULL	0	NULL	Upc2p	GP		bind					ERG2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6395_s_287	11533229	(A) The 7-bp sequence TCGTATA was necessary for Upc2p binding to the  ERG2 promoter.	bind
7923	2	3223	5	11	NULL	0	NULL				is necessary for				TCGTATA	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6395_s_287	11533229	(A) The 7-bp sequence TCGTATA was necessary for Upc2p binding to the  ERG2 promoter.	bind
9526	1	3223	7	11	NULL	0	NULL	Upc2p	GP		bind					ERG2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6395_s_287	11533229	(A) The 7-bp sequence TCGTATA was necessary for Upc2p binding to the  ERG2 promoter.	bind
9527	2	3223	7	11	NULL	0	NULL				is necessary for				TCGTATA	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6395_s_287	11533229	(A) The 7-bp sequence TCGTATA was necessary for Upc2p binding to the  ERG2 promoter.	bind
80120	1	3223	11	NULL	NULL	0	NULL	Upc2p	GeneOrProtein		binds to 					ERG2 promoter	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_19_6395_s_287	11533229	(A) The 7-bp sequence TCGTATA was necessary for Upc2p binding to the  ERG2 promoter.	bind
80121	2	3223	11	NULL	NULL	0	NULL	Upc2p	Gene		is  necessary for				TCGTATA	statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_19_6395_s_287	11533229	(A) The 7-bp sequence TCGTATA was necessary for Upc2p binding to the  ERG2 promoter.	bind
7924	1	3227	5	11	NULL	0	NULL	MAPs	GP	addition of	restore					aster 	CellComponent	formation of			NULL	deltaRanBPdeltaAPA extract	NULL	NULL	NULL	NULL	gw60_cell_104_1_95_s_209	11163243	(A) The addition of MAPs or importin beta binding  proteins can restore aster formation in the deltaRanBPdeltaAPA extract.	bind
7925	2	3227	5	11	NULL	0	NULL	importin beta binding protein	GP	addition of	restore					aster 	CellComponent	formation of			NULL	deltaRanBPdeltaAPA extract	NULL	NULL	NULL	NULL	gw60_cell_104_1_95_s_209	11163243	(A) The addition of MAPs or importin beta binding  proteins can restore aster formation in the deltaRanBPdeltaAPA extract.	bind
9529	1	3227	7	11	NULL	0	NULL	MAPs	GP	addition of	restore					aster	CellComponent	formation of			NULL	deltaRanBPdeltaAPA extract	NULL	NULL	NULL	NULL	gw60_cell_104_1_95_s_209	11163243	(A) The addition of MAPs or importin beta binding  proteins can restore aster formation in the deltaRanBPdeltaAPA extract.	bind
9530	2	3227	7	11	NULL	0	NULL	importin beta binding proteins	GP	addition of	restore					aster	CellComponent	formation of			NULL	deltaRanBPdeltaAPA extract	NULL	NULL	NULL	NULL	gw60_cell_104_1_95_s_209	11163243	(A) The addition of MAPs or importin beta binding  proteins can restore aster formation in the deltaRanBPdeltaAPA extract.	bind
80122	1	3227	11	NULL	NULL	0	NULL	deltaRanBPdeltaAPA extract	Thing		can form					aster	CellComponent				NULL		0	NULL	NULL	NULL	gw60_cell_104_1_95_s_209	11163243	(A) The addition of MAPs or importin beta binding  proteins can restore aster formation in the deltaRanBPdeltaAPA extract.	bind
80123	2	3227	11	NULL	NULL	0	NULL	MAPs	Protein		can restore					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_cell_104_1_95_s_209	11163243	(A) The addition of MAPs or importin beta binding  proteins can restore aster formation in the deltaRanBPdeltaAPA extract.	bind
80124	3	3227	11	NULL	NULL	0	NULL	importin beta binding proteins	Protein		can restore					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_cell_104_1_95_s_209	11163243	(A) The addition of MAPs or importin beta binding  proteins can restore aster formation in the deltaRanBPdeltaAPA extract.	bind
7927	1	3229	5	11	NULL	0	NULL	Galpha	GP		bind			alphaN domain		receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4557_s_45	16030250	(A) The alphaN domain provides one of the binding interfaces between Galpha and Gbeta and the receptor.	bind
7928	2	3229	5	11	NULL	0	NULL	Gbeta	GP		bind			alphaN domain		receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4557_s_45	16030250	(A) The alphaN domain provides one of the binding interfaces between Galpha and Gbeta and the receptor.	bind
9531	1	3229	7	11	NULL	0	NULL	Galpha 	GP		bind			alphaN domain		receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4557_s_45	16030250	(A) The alphaN domain provides one of the binding interfaces between Galpha and Gbeta and the receptor.	bind
9532	2	3229	7	11	NULL	0	NULL	Gbeta	GP		bind			alphaN domain		receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4557_s_45	16030250	(A) The alphaN domain provides one of the binding interfaces between Galpha and Gbeta and the receptor.	bind
80125	1	3229	11	NULL	NULL	NULL	NULL	Galpha	Protein		binds to 			alphaN domain		receptor	Protein				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4557_s_45	16030250	(A) The alphaN domain provides one of the binding interfaces between Galpha and Gbeta and the receptor.	bind
80126	2	3229	11	NULL	NULL	0	NULL	Gbeta	Protein		binds to 					receptor	Protein				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4557_s_45	16030250	(A) The alphaN domain provides one of the binding interfaces between Galpha and Gbeta and the receptor.	bind
7931	1	3232	5	11	NULL	0	NULL	ATM	GP		bind					linear plasmid DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5363_s_319	15964794	(A) The anti-C147 antibodies prevent ATM binding to the linear plasmid DNA.	bind
7932	2	3232	5	11	NULL	0	NULL	anti-C147 antibodies	GP		prevent					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5363_s_319	15964794	(A) The anti-C147 antibodies prevent ATM binding to the linear plasmid DNA.	bind
9533	1	3232	7	11	NULL	0	NULL	ATM	GP		bind					linear plasmid DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5363_s_319	15964794	(A) The anti-C147 antibodies prevent ATM binding to the linear plasmid DNA.	bind
9534	2	3232	7	11	NULL	0	NULL	anti-C147 antibodies	GP		prevent					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5363_s_319	15964794	(A) The anti-C147 antibodies prevent ATM binding to the linear plasmid DNA.	bind
80127	1	3232	11	NULL	NULL	0	NULL	ATM	Protein		binds to 					DNA	NucleicAcidSubstance	linear plasmid			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_13_5363_s_319	15964794	(A) The anti-C147 antibodies prevent ATM binding to the linear plasmid DNA.	bind
80128	2	3232	11	NULL	NULL	0	NULL	anti-C147 antibodies	PartOfProtein		prevents					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_13_5363_s_319	15964794	(A) The anti-C147 antibodies prevent ATM binding to the linear plasmid DNA.	bind
8195	1	3233	5	11	NULL	0	NULL	anti-VapA	GP		reacted with					VapA	GP				NULL	in SRA	NULL	NULL	NULL	NULL	gw70_infectimmun_71_11_6329_s_74	14573652	(A) The anti-VapA monoclonal antibody reacted with  VapA in SRA and the pellet antigen and six protein bands in the CFS antigen.	bind
8196	2	3233	5	11	NULL	0	NULL	anti-VapA	GP		reacted with					pellet antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_71_11_6329_s_74	14573652	(A) The anti-VapA monoclonal antibody reacted with  VapA in SRA and the pellet antigen and six protein bands in the CFS antigen.	bind
8197	3	3233	5	11	NULL	0	NULL	anti-VapA	GP		reacted with					six protein bands	GP				NULL	in CFS antigen	NULL	NULL	NULL	NULL	gw70_infectimmun_71_11_6329_s_74	14573652	(A) The anti-VapA monoclonal antibody reacted with  VapA in SRA and the pellet antigen and six protein bands in the CFS antigen.	bind
44748	4	3233	5	11	NULL	0	NULL	anti-VapA	GP		is a type of					monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_71_11_6329_s_74	14573652	(A) The anti-VapA monoclonal antibody reacted with  VapA in SRA and the pellet antigen and six protein bands in the CFS antigen.	bind
9535	1	3233	7	11	NULL	0	NULL	 anti-VapA 	GP		reacts with					VapA	GP				NULL	in SRA	NULL	NULL	NULL	NULL	gw70_infectimmun_71_11_6329_s_74	14573652	(A) The anti-VapA monoclonal antibody reacted with  VapA in SRA and the pellet antigen and six protein bands in the CFS antigen.	bind
9925	2	3233	7	11	NULL	0	NULL	anti-VapA	GP		reacts with					pellet antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_71_11_6329_s_74	14573652	(A) The anti-VapA monoclonal antibody reacted with  VapA in SRA and the pellet antigen and six protein bands in the CFS antigen.	bind
12378	3	3233	7	11	NULL	0	NULL	anti-VapA	GP		reacts with					six protein bands 	GP				NULL	CFS antigen	NULL	NULL	NULL	NULL	gw70_infectimmun_71_11_6329_s_74	14573652	(A) The anti-VapA monoclonal antibody reacted with  VapA in SRA and the pellet antigen and six protein bands in the CFS antigen.	bind
44749	4	3233	7	11	NULL	0	NULL	anti-VapA	GP		is a type of					monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_71_11_6329_s_74	14573652	(A) The anti-VapA monoclonal antibody reacted with  VapA in SRA and the pellet antigen and six protein bands in the CFS antigen.	bind
80129	1	3233	11	NULL	NULL	0	NULL	anti-VapA	PartOfProtein	monoclonal antibody	reacted with					VapA	Protein	in SRA			NULL		0	NULL	NULL	NULL	gw70_infectimmun_71_11_6329_s_74	14573652	(A) The anti-VapA monoclonal antibody reacted with  VapA in SRA and the pellet antigen and six protein bands in the CFS antigen.	bind
7933	1	3234	5	11	NULL	0	NULL	LexA-Snf1	GP		bind					lacZ reporter	NucleicAcid			LexA sites 5' to promoter of	NULL		NULL	NULL	NULL	NULL	gw60_genetics_163_2_507_s_147	12618390	(A) The assay for kinase activity entails binding of LexA-Snf1 to LexA sites 5' to the promoter of a  lacZ reporter.	bind
9552	1	3234	7	11	NULL	0	NULL	LexA-Snf1	GP		bind					lacZ reporter	NucleicAcid			LexA sites 5' to the promoter of	NULL		NULL	NULL	NULL	NULL	gw60_genetics_163_2_507_s_147	12618390	(A) The assay for kinase activity entails binding of LexA-Snf1 to LexA sites 5' to the promoter of a  lacZ reporter.	bind
80130	1	3234	11	NULL	NULL	NULL	NULL	LexA-Snf1	Protein		binds to 					LexA	Gene			sites 5'	NULL		NULL	NULL	NULL	NULL	gw60_genetics_163_2_507_s_147	12618390	(A) The assay for kinase activity entails binding of LexA-Snf1 to LexA sites 5' to the promoter of a  lacZ reporter.	bind
80131	2	3234	11	NULL	NULL	0	NULL	statement 1	Protein		binds to 					lacZ reporter	Gene	promoter			NULL		0	NULL	NULL	NULL	gw60_genetics_163_2_507_s_147	12618390	(A) The assay for kinase activity entails binding of LexA-Snf1 to LexA sites 5' to the promoter of a  lacZ reporter.	bind
7934	1	3236	5	11	NULL	0	NULL	BTAF1	GP	ATPase-deficient;; mutant	bind					TBP	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_22_10072_s_122	15509807	(A) The ATPase-deficient mutant of BTAF1 binds to TBP in the presence of NC2alpha.	bind
7935	2	3236	5	11	NULL	0	NULL	statement 1	Process		in the presence of					NC2alpha	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_22_10072_s_122	15509807	(A) The ATPase-deficient mutant of BTAF1 binds to TBP in the presence of NC2alpha.	bind
9553	1	3236	7	11	NULL	0	NULL	BTAF1	GP	ATPase-deficient;; mutant	bind					TBP	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_22_10072_s_122	15509807	(A) The ATPase-deficient mutant of BTAF1 binds to TBP in the presence of NC2alpha.	bind
9554	2	3236	7	11	NULL	0	NULL	statement 1	Process		occurs in the presence of					NC2alpha	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_22_10072_s_122	15509807	(A) The ATPase-deficient mutant of BTAF1 binds to TBP in the presence of NC2alpha.	bind
80132	1	3236	11	NULL	NULL	0	NULL	BTAF1	GeneOrProtein	 ATPase-deficient mutant	binds to 					TBP	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_22_10072_s_122	15509807	(A) The ATPase-deficient mutant of BTAF1 binds to TBP in the presence of NC2alpha.	bind
80133	2	3236	11	NULL	NULL	0	NULL	statement 1	Process		occurs in the presence of					NC2alpha	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_22_10072_s_122	15509807	(A) The ATPase-deficient mutant of BTAF1 binds to TBP in the presence of NC2alpha.	bind
7937	1	3238	5	11	NULL	0	NULL	Pho4p	GP		bind			helix-loop-helix domain		DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_yeast_19_7_641_s_154	11967834	(A) The basic helix-loop-helix domain  from Pho4p bound to DNA (PDB Accession No. 1A0A).	bind
9555	1	3238	7	11	NULL	0	NULL	Pho4p	GP		bind			basic helix-loop-helix		DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_yeast_19_7_641_s_154	11967834	(A) The basic helix-loop-helix domain  from Pho4p bound to DNA (PDB Accession No. 1A0A).	bind
80134	1	3238	11	NULL	NULL	0	NULL	Pho4p	Protein		binds to 			helix-loop-helix domain		DNA	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_yeast_19_7_641_s_154	11967834	(A) The basic helix-loop-helix domain  from Pho4p bound to DNA (PDB Accession No. 1A0A).	bind
7938	1	3239	5	11	NULL	0	NULL	ASK1	GP		bind					TRAF2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2198_s_118	10688666	(A) The binding of ASK1 and TRAF2 involves the amino-terminal (aa 1 to 460) and carboxyl-terminal (aa 937 to 1375) noncatalytic domains of ASK1.	bind
7940	2	3239	5	11	NULL	0	NULL	statement 1	Process		involves					ASK1	GP	noncatalytic domain	amino-terminal (aa 1 to 460)		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2198_s_118	10688666	(A) The binding of ASK1 and TRAF2 involves the amino-terminal (aa 1 to 460) and carboxyl-terminal (aa 937 to 1375) noncatalytic domains of ASK1.	bind
7941	3	3239	5	11	NULL	0	NULL	statement 1	Process		involves					ASK1	GP	noncatalytic domain	carboxyl-terminal (aa 937 to 1375)		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2198_s_118	10688666	(A) The binding of ASK1 and TRAF2 involves the amino-terminal (aa 1 to 460) and carboxyl-terminal (aa 937 to 1375) noncatalytic domains of ASK1.	bind
9556	1	3239	7	11	NULL	0	NULL	ASK1	GP		bind					TRAF2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2198_s_118	10688666	(A) The binding of ASK1 and TRAF2 involves the amino-terminal (aa 1 to 460) and carboxyl-terminal (aa 937 to 1375) noncatalytic domains of ASK1.	bind
12379	2	3239	7	11	NULL	0	NULL	statement 1	Process		involves					ASK1	GP	noncatalytic	amino-terminal aa 1 to 460		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2198_s_118	10688666	(A) The binding of ASK1 and TRAF2 involves the amino-terminal (aa 1 to 460) and carboxyl-terminal (aa 937 to 1375) noncatalytic domains of ASK1.	bind
12380	3	3239	7	11	NULL	0	NULL	statement 1	Process		involves					ASK1	GP	noncatalytic	carboxyl-terminal aa 937 to 1375		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2198_s_118	10688666	(A) The binding of ASK1 and TRAF2 involves the amino-terminal (aa 1 to 460) and carboxyl-terminal (aa 937 to 1375) noncatalytic domains of ASK1.	bind
80135	1	3239	11	NULL	NULL	0	NULL	ASK1	Protein		binds to 			amino-terminal (aa 1 to 460);;carboxyl-terminal (aa 937 to 1375)		TRAF2	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_6_2198_s_118	10688666	(A) The binding of ASK1 and TRAF2 involves the amino-terminal (aa 1 to 460) and carboxyl-terminal (aa 937 to 1375) noncatalytic domains of ASK1.	bind
8198	1	3241	5	11	NULL	0	NULL	DDP1	GP		bind					oligo 6Rc	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_11_3860_s_198	10805729	(A) The binding of DDP1 and 1/2DDP1 to oligo 6Rc (panels 6Rc), oligo 9Rc (panels 9Rc), oligo 9R (panels 9R), fragment 12R (panels 12R), and fragment 42R (panels 42R) is presented as a function of increasing protein concentrations: a threefold-higher protein concentration was used in lanes 2 than in lanes 1.	bind
8199	2	3241	5	11	NULL	0	NULL	DDP1	GP		bind					oligo 9Rc	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_11_3860_s_198	10805729	(A) The binding of DDP1 and 1/2DDP1 to oligo 6Rc (panels 6Rc), oligo 9Rc (panels 9Rc), oligo 9R (panels 9R), fragment 12R (panels 12R), and fragment 42R (panels 42R) is presented as a function of increasing protein concentrations: a threefold-higher protein concentration was used in lanes 2 than in lanes 1.	bind
8200	3	3241	5	11	NULL	0	NULL	DDP1	GP		bind					oligo 9R	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_11_3860_s_198	10805729	(A) The binding of DDP1 and 1/2DDP1 to oligo 6Rc (panels 6Rc), oligo 9Rc (panels 9Rc), oligo 9R (panels 9R), fragment 12R (panels 12R), and fragment 42R (panels 42R) is presented as a function of increasing protein concentrations: a threefold-higher protein concentration was used in lanes 2 than in lanes 1.	bind
8201	4	3241	5	11	NULL	0	NULL	DDP1	GP		bind					fragment 12R	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_11_3860_s_198	10805729	(A) The binding of DDP1 and 1/2DDP1 to oligo 6Rc (panels 6Rc), oligo 9Rc (panels 9Rc), oligo 9R (panels 9R), fragment 12R (panels 12R), and fragment 42R (panels 42R) is presented as a function of increasing protein concentrations: a threefold-higher protein concentration was used in lanes 2 than in lanes 1.	bind
8202	5	3241	5	11	NULL	0	NULL	DDP1	GP		bind					fragment 42R	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_11_3860_s_198	10805729	(A) The binding of DDP1 and 1/2DDP1 to oligo 6Rc (panels 6Rc), oligo 9Rc (panels 9Rc), oligo 9R (panels 9R), fragment 12R (panels 12R), and fragment 42R (panels 42R) is presented as a function of increasing protein concentrations: a threefold-higher protein concentration was used in lanes 2 than in lanes 1.	bind
9926	1	3241	7	11	NULL	0	NULL	 DDP1	GP		bind					oligo 6Rc	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_11_3860_s_198	10805729	(A) The binding of DDP1 and 1/2DDP1 to oligo 6Rc (panels 6Rc), oligo 9Rc (panels 9Rc), oligo 9R (panels 9R), fragment 12R (panels 12R), and fragment 42R (panels 42R) is presented as a function of increasing protein concentrations: a threefold-higher protein concentration was used in lanes 2 than in lanes 1.	bind
9927	2	3241	7	11	NULL	0	NULL	DDP1	GP		bind					oligo 9Rc	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_11_3860_s_198	10805729	(A) The binding of DDP1 and 1/2DDP1 to oligo 6Rc (panels 6Rc), oligo 9Rc (panels 9Rc), oligo 9R (panels 9R), fragment 12R (panels 12R), and fragment 42R (panels 42R) is presented as a function of increasing protein concentrations: a threefold-higher protein concentration was used in lanes 2 than in lanes 1.	bind
9928	3	3241	7	11	NULL	0	NULL	DDP1	GP		bind					oligo 9R	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_11_3860_s_198	10805729	(A) The binding of DDP1 and 1/2DDP1 to oligo 6Rc (panels 6Rc), oligo 9Rc (panels 9Rc), oligo 9R (panels 9R), fragment 12R (panels 12R), and fragment 42R (panels 42R) is presented as a function of increasing protein concentrations: a threefold-higher protein concentration was used in lanes 2 than in lanes 1.	bind
9929	4	3241	7	11	NULL	0	NULL	DDP1	GP		bind					fragment 12R	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_11_3860_s_198	10805729	(A) The binding of DDP1 and 1/2DDP1 to oligo 6Rc (panels 6Rc), oligo 9Rc (panels 9Rc), oligo 9R (panels 9R), fragment 12R (panels 12R), and fragment 42R (panels 42R) is presented as a function of increasing protein concentrations: a threefold-higher protein concentration was used in lanes 2 than in lanes 1.	bind
9930	5	3241	7	11	NULL	0	NULL	DDP1	GP		bind					fragment 42R	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_11_3860_s_198	10805729	(A) The binding of DDP1 and 1/2DDP1 to oligo 6Rc (panels 6Rc), oligo 9Rc (panels 9Rc), oligo 9R (panels 9R), fragment 12R (panels 12R), and fragment 42R (panels 42R) is presented as a function of increasing protein concentrations: a threefold-higher protein concentration was used in lanes 2 than in lanes 1.	bind
80147	1	3241	11	NULL	NULL	0	NULL	DDP1	Protein		binds to 					 oligo 6Rc	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_11_3860_s_198	10805729	(A) The binding of DDP1 and 1/2DDP1 to oligo 6Rc (panels 6Rc), oligo 9Rc (panels 9Rc), oligo 9R (panels 9R), fragment 12R (panels 12R), and fragment 42R (panels 42R) is presented as a function of increasing protein concentrations: a threefold-higher protein concentration was used in lanes 2 than in lanes 1.	bind
80148	2	3241	11	NULL	NULL	0	NULL	DDP1	Protein		binds to 					oligo 9Rc	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_11_3860_s_198	10805729	(A) The binding of DDP1 and 1/2DDP1 to oligo 6Rc (panels 6Rc), oligo 9Rc (panels 9Rc), oligo 9R (panels 9R), fragment 12R (panels 12R), and fragment 42R (panels 42R) is presented as a function of increasing protein concentrations: a threefold-higher protein concentration was used in lanes 2 than in lanes 1.	bind
80149	3	3241	11	NULL	NULL	0	NULL	DDP1	Protein		binds to 					 oligo 9R	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_11_3860_s_198	10805729	(A) The binding of DDP1 and 1/2DDP1 to oligo 6Rc (panels 6Rc), oligo 9Rc (panels 9Rc), oligo 9R (panels 9R), fragment 12R (panels 12R), and fragment 42R (panels 42R) is presented as a function of increasing protein concentrations: a threefold-higher protein concentration was used in lanes 2 than in lanes 1.	bind
80150	4	3241	11	NULL	NULL	0	NULL	 DDP1	Protein		binds to 					fragment 12R	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_11_3860_s_198	10805729	(A) The binding of DDP1 and 1/2DDP1 to oligo 6Rc (panels 6Rc), oligo 9Rc (panels 9Rc), oligo 9R (panels 9R), fragment 12R (panels 12R), and fragment 42R (panels 42R) is presented as a function of increasing protein concentrations: a threefold-higher protein concentration was used in lanes 2 than in lanes 1.	bind
80151	5	3241	11	NULL	NULL	0	NULL	DDP1	Protein		binds to 					fragment 42R	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_11_3860_s_198	10805729	(A) The binding of DDP1 and 1/2DDP1 to oligo 6Rc (panels 6Rc), oligo 9Rc (panels 9Rc), oligo 9R (panels 9R), fragment 12R (panels 12R), and fragment 42R (panels 42R) is presented as a function of increasing protein concentrations: a threefold-higher protein concentration was used in lanes 2 than in lanes 1.	bind
80152	6	3241	11	NULL	NULL	NULL	NULL	1/2DDP1	Protein		binds to 					oligo 6Rc	NucleicAcidSubstance				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_11_3860_s_198	10805729	(A) The binding of DDP1 and 1/2DDP1 to oligo 6Rc (panels 6Rc), oligo 9Rc (panels 9Rc), oligo 9R (panels 9R), fragment 12R (panels 12R), and fragment 42R (panels 42R) is presented as a function of increasing protein concentrations: a threefold-higher protein concentration was used in lanes 2 than in lanes 1.	bind
80153	7	3241	11	NULL	NULL	0	NULL	1/2DDP1	Protein		binds to 					oligo 9Rc 	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_11_3860_s_198	10805729	(A) The binding of DDP1 and 1/2DDP1 to oligo 6Rc (panels 6Rc), oligo 9Rc (panels 9Rc), oligo 9R (panels 9R), fragment 12R (panels 12R), and fragment 42R (panels 42R) is presented as a function of increasing protein concentrations: a threefold-higher protein concentration was used in lanes 2 than in lanes 1.	bind
80154	8	3241	11	NULL	NULL	0	NULL	1/2DDP1	Protein		binds to 					oligo 9Rc	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_11_3860_s_198	10805729	(A) The binding of DDP1 and 1/2DDP1 to oligo 6Rc (panels 6Rc), oligo 9Rc (panels 9Rc), oligo 9R (panels 9R), fragment 12R (panels 12R), and fragment 42R (panels 42R) is presented as a function of increasing protein concentrations: a threefold-higher protein concentration was used in lanes 2 than in lanes 1.	bind
80155	9	3241	11	NULL	NULL	0	NULL	1/2DDP1	Protein		binds to 					fragment 12R	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_11_3860_s_198	10805729	(A) The binding of DDP1 and 1/2DDP1 to oligo 6Rc (panels 6Rc), oligo 9Rc (panels 9Rc), oligo 9R (panels 9R), fragment 12R (panels 12R), and fragment 42R (panels 42R) is presented as a function of increasing protein concentrations: a threefold-higher protein concentration was used in lanes 2 than in lanes 1.	bind
80156	10	3241	11	NULL	NULL	0	NULL	1/2DDP1	Protein		binds to 					fragment 42R	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_11_3860_s_198	10805729	(A) The binding of DDP1 and 1/2DDP1 to oligo 6Rc (panels 6Rc), oligo 9Rc (panels 9Rc), oligo 9R (panels 9R), fragment 12R (panels 12R), and fragment 42R (panels 42R) is presented as a function of increasing protein concentrations: a threefold-higher protein concentration was used in lanes 2 than in lanes 1.	bind
7942	1	3242	5	11	NULL	0	NULL	GST-LSP1 fusion proteins	GP		bind					F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1642_1_17_s_86	12972289	(A) The binding of GST and  the indicated GST-LSP1 fusion proteins to F-actin was determined in a high-speed  co-sedimentation assay.	bind
7943	2	3242	5	11	NULL	0	NULL	GST	GP		bind					F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1642_1_17_s_86	12972289	(A) The binding of GST and  the indicated GST-LSP1 fusion proteins to F-actin was determined in a high-speed  co-sedimentation assay.	bind
9931	1	3242	7	11	NULL	0	NULL	GST	GP		bind					F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1642_1_17_s_86	12972289	(A) The binding of GST and  the indicated GST-LSP1 fusion proteins to F-actin was determined in a high-speed  co-sedimentation assay.	bind
9932	2	3242	7	11	NULL	0	NULL	GST-LSP1	GP		bind					F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1642_1_17_s_86	12972289	(A) The binding of GST and  the indicated GST-LSP1 fusion proteins to F-actin was determined in a high-speed  co-sedimentation assay.	bind
80157	1	3242	11	NULL	NULL	0	NULL	GST	Protein		binds to 					F-actin	Protein				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1642_1_17_s_86	12972289	(A) The binding of GST and  the indicated GST-LSP1 fusion proteins to F-actin was determined in a high-speed  co-sedimentation assay.	bind
80158	2	3242	11	NULL	NULL	0	NULL	GST-LSP1	Protein		binds to 					F-actin	Protein				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1642_1_17_s_86	12972289	(A) The binding of GST and  the indicated GST-LSP1 fusion proteins to F-actin was determined in a high-speed  co-sedimentation assay.	bind
80159	3	3242	11	NULL	NULL	0	NULL	high-speed co-sedimentation assay	ResearchActivity		determines					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1642_1_17_s_86	12972289	(A) The binding of GST and  the indicated GST-LSP1 fusion proteins to F-actin was determined in a high-speed  co-sedimentation assay.	bind
80160	4	3242	11	NULL	NULL	0	NULL	high-speed co-sedimentation assay	ResearchActivity		determines					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1642_1_17_s_86	12972289	(A) The binding of GST and  the indicated GST-LSP1 fusion proteins to F-actin was determined in a high-speed  co-sedimentation assay.	bind
8015	1	3244	5	11	NULL	0	NULL	MutS	GP		bind									ICLs	NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_1_71_s_144	12943665	(A) The binding of MutS   to ICLs is stimulated by PCNA, (B) a DNA helicase in cooperation with RPA creates  a bubble or open region proximate to the ICL. Ercc1-Xpf is recruited to the site  and forms incisions on either side of the lesion as shown in (C).	bind
8016	2	3244	5	11	NULL	0	NULL	PCNA	GP		stimulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_1_71_s_144	12943665	(A) The binding of MutS   to ICLs is stimulated by PCNA, (B) a DNA helicase in cooperation with RPA creates  a bubble or open region proximate to the ICL. Ercc1-Xpf is recruited to the site  and forms incisions on either side of the lesion as shown in (C).	bind
8017	3	3244	5	11	NULL	0	NULL	DNA helicase	GP		creates					open region	NucleicAcid	proximate to 		ICL	NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_1_71_s_144	12943665	(A) The binding of MutS   to ICLs is stimulated by PCNA, (B) a DNA helicase in cooperation with RPA creates  a bubble or open region proximate to the ICL. Ercc1-Xpf is recruited to the site  and forms incisions on either side of the lesion as shown in (C).	bind
8018	4	3244	5	11	NULL	0	NULL	RPA	GP		creates					open region	NucleicAcid	proximate to		ICL	NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_1_71_s_144	12943665	(A) The binding of MutS   to ICLs is stimulated by PCNA, (B) a DNA helicase in cooperation with RPA creates  a bubble or open region proximate to the ICL. Ercc1-Xpf is recruited to the site  and forms incisions on either side of the lesion as shown in (C).	bind
8019	5	3244	5	11	NULL	0	NULL	statement 3	Process		occurs in cooperation with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_1_71_s_144	12943665	(A) The binding of MutS   to ICLs is stimulated by PCNA, (B) a DNA helicase in cooperation with RPA creates  a bubble or open region proximate to the ICL. Ercc1-Xpf is recruited to the site  and forms incisions on either side of the lesion as shown in (C).	bind
9933	1	3244	7	11	NULL	0	NULL	MutS	GP		bind					ICLs	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_1_71_s_144	12943665	(A) The binding of MutS   to ICLs is stimulated by PCNA, (B) a DNA helicase in cooperation with RPA creates  a bubble or open region proximate to the ICL. Ercc1-Xpf is recruited to the site  and forms incisions on either side of the lesion as shown in (C).	bind
9934	2	3244	7	11	NULL	0	NULL	statement 1	Process		is stimulated by					PCNA	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_1_71_s_144	12943665	(A) The binding of MutS   to ICLs is stimulated by PCNA, (B) a DNA helicase in cooperation with RPA creates  a bubble or open region proximate to the ICL. Ercc1-Xpf is recruited to the site  and forms incisions on either side of the lesion as shown in (C).	bind
9935	3	3244	7	11	NULL	0	NULL	DNA helicase	GP		creates					open region	NucleicAcid	proximate to		ICL	NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_1_71_s_144	12943665	(A) The binding of MutS   to ICLs is stimulated by PCNA, (B) a DNA helicase in cooperation with RPA creates  a bubble or open region proximate to the ICL. Ercc1-Xpf is recruited to the site  and forms incisions on either side of the lesion as shown in (C).	bind
9936	4	3244	7	11	NULL	0	NULL	RPA	GP		creates					 open region	NucleicAcid	proximate to		ICL	NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_1_71_s_144	12943665	(A) The binding of MutS   to ICLs is stimulated by PCNA, (B) a DNA helicase in cooperation with RPA creates  a bubble or open region proximate to the ICL. Ercc1-Xpf is recruited to the site  and forms incisions on either side of the lesion as shown in (C).	bind
9937	5	3244	7	11	NULL	0	NULL	statement 3	Process		occurs in cooperation with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_1_71_s_144	12943665	(A) The binding of MutS   to ICLs is stimulated by PCNA, (B) a DNA helicase in cooperation with RPA creates  a bubble or open region proximate to the ICL. Ercc1-Xpf is recruited to the site  and forms incisions on either side of the lesion as shown in (C).	bind
80161	1	3244	11	NULL	NULL	0	NULL	MutS	Protein		binds to 					ICLs	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_1_71_s_144	12943665	(A) The binding of MutS   to ICLs is stimulated by PCNA, (B) a DNA helicase in cooperation with RPA creates  a bubble or open region proximate to the ICL. Ercc1-Xpf is recruited to the site  and forms incisions on either side of the lesion as shown in (C).	bind
80162	2	3244	11	NULL	NULL	0	NULL	PCNA	Protein		stimulates					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_1_71_s_144	12943665	(A) The binding of MutS   to ICLs is stimulated by PCNA, (B) a DNA helicase in cooperation with RPA creates  a bubble or open region proximate to the ICL. Ercc1-Xpf is recruited to the site  and forms incisions on either side of the lesion as shown in (C).	bind
80163	3	3244	11	NULL	NULL	NULL	NULL	PCNA	Protein		creates					bubble	NucleicAcidSubstance	proximate to the ICL			NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_1_71_s_144	12943665	(A) The binding of MutS   to ICLs is stimulated by PCNA, (B) a DNA helicase in cooperation with RPA creates  a bubble or open region proximate to the ICL. Ercc1-Xpf is recruited to the site  and forms incisions on either side of the lesion as shown in (C).	bind
80164	4	3244	11	NULL	NULL	0	NULL	RPA	Protein		creates					bubble	NucleicAcidSubstance	proximate to the ICL			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_1_71_s_144	12943665	(A) The binding of MutS   to ICLs is stimulated by PCNA, (B) a DNA helicase in cooperation with RPA creates  a bubble or open region proximate to the ICL. Ercc1-Xpf is recruited to the site  and forms incisions on either side of the lesion as shown in (C).	bind
80165	5	3244	11	NULL	NULL	0	NULL	PCNA	Protein		is a type of 					DNA helicase	Protein				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_1_71_s_144	12943665	(A) The binding of MutS   to ICLs is stimulated by PCNA, (B) a DNA helicase in cooperation with RPA creates  a bubble or open region proximate to the ICL. Ercc1-Xpf is recruited to the site  and forms incisions on either side of the lesion as shown in (C).	bind
80166	6	3244	11	NULL	NULL	0	NULL	PCNA	Protein		creates					open region	NucleicAcidSubstance	proximate to the ICL			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_1_71_s_144	12943665	(A) The binding of MutS   to ICLs is stimulated by PCNA, (B) a DNA helicase in cooperation with RPA creates  a bubble or open region proximate to the ICL. Ercc1-Xpf is recruited to the site  and forms incisions on either side of the lesion as shown in (C).	bind
80167	7	3244	11	NULL	NULL	0	NULL	RPA	Protein		creates					open region	NucleicAcidSubstance	proximate to the ICL			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_1_71_s_144	12943665	(A) The binding of MutS   to ICLs is stimulated by PCNA, (B) a DNA helicase in cooperation with RPA creates  a bubble or open region proximate to the ICL. Ercc1-Xpf is recruited to the site  and forms incisions on either side of the lesion as shown in (C).	bind
80168	8	3244	11	NULL	NULL	0	NULL	statement 3	Process		occurs along with					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_1_71_s_144	12943665	(A) The binding of MutS   to ICLs is stimulated by PCNA, (B) a DNA helicase in cooperation with RPA creates  a bubble or open region proximate to the ICL. Ercc1-Xpf is recruited to the site  and forms incisions on either side of the lesion as shown in (C).	bind
80169	9	3244	11	NULL	NULL	0	NULL	statement 6	Process		occurs along with					statement 7	Process				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_1_71_s_144	12943665	(A) The binding of MutS   to ICLs is stimulated by PCNA, (B) a DNA helicase in cooperation with RPA creates  a bubble or open region proximate to the ICL. Ercc1-Xpf is recruited to the site  and forms incisions on either side of the lesion as shown in (C).	bind
80170	10	3244	11	NULL	NULL	0	NULL	Ercc1-Xpf	Protein		forms					incisions					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_1_71_s_144	12943665	(A) The binding of MutS   to ICLs is stimulated by PCNA, (B) a DNA helicase in cooperation with RPA creates  a bubble or open region proximate to the ICL. Ercc1-Xpf is recruited to the site  and forms incisions on either side of the lesion as shown in (C).	bind
8022	1	3246	5	11	NULL	0	NULL	p65	GP		bind					IkappaBalpha	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_3_1113_s_269	15657437	(A) The binding of p65 to the  IkappaBalpha promoter is increased in  Pias1 null cells.	bind
8023	2	3246	5	11	NULL	0	NULL	statement 1	Process		is increased in					Pias1 null cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_3_1113_s_269	15657437	(A) The binding of p65 to the  IkappaBalpha promoter is increased in  Pias1 null cells.	bind
9938	1	3246	7	11	NULL	0	NULL	p65	GP		binds					IkappaBalpha	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_3_1113_s_269	15657437	(A) The binding of p65 to the  IkappaBalpha promoter is increased in  Pias1 null cells.	bind
9939	2	3246	7	11	NULL	0	NULL	statement 1	Process		is increased in					Pias1 null cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_3_1113_s_269	15657437	(A) The binding of p65 to the  IkappaBalpha promoter is increased in  Pias1 null cells.	bind
80171	1	3246	11	NULL	NULL	0	NULL	p65	Protein		binds to 					IkappaBalpha promoter	Gene				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_3_1113_s_269	15657437	(A) The binding of p65 to the  IkappaBalpha promoter is increased in  Pias1 null cells.	bind
80172	2	3246	11	NULL	NULL	0	NULL	statement 1	Process		increased in					Pias1 null cells	Cell				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_3_1113_s_269	15657437	(A) The binding of p65 to the  IkappaBalpha promoter is increased in  Pias1 null cells.	bind
8024	1	3247	5	11	NULL	0	NULL	S-CDK	GP	binding of	restrict					Sic1	GP	ubiquitination of;; number of	lysines		NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_6_1435_s_163	12820958	(A) The binding of S-CDK restricts the number of lysines in Sic1 that can be ubiquitinated.	bind
9941	1	3247	7	11	NULL	0	NULL	S-CDK	GP	binding of	restricts					Sic1	GP	ubiquitination of;; number of	lysine		NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_6_1435_s_163	12820958	(A) The binding of S-CDK restricts the number of lysines in Sic1 that can be ubiquitinated.	bind
80173	1	3247	11	NULL	NULL	0	NULL	S-CDK	Protein		binds to 					Sic1	Protein				NULL		0	NULL	NULL	NULL	gw60_molcell_11_6_1435_s_163	12820958	(A) The binding of S-CDK restricts the number of lysines in Sic1 that can be ubiquitinated.	bind
80174	2	3247	11	NULL	NULL	0	NULL	 lysines	AminoAcid	in Sic1	 can be					ubiquitinated	MolecularProcess				NULL		0	NULL	NULL	NULL	gw60_molcell_11_6_1435_s_163	12820958	(A) The binding of S-CDK restricts the number of lysines in Sic1 that can be ubiquitinated.	bind
80175	3	3247	11	NULL	NULL	0	NULL	statement 1	Process		 restricts					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_11_6_1435_s_163	12820958	(A) The binding of S-CDK restricts the number of lysines in Sic1 that can be ubiquitinated.	bind
8025	1	3248	5	11	NULL	0	NULL	SPN	GP		bind					importin-beta	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4660_s_261	16030253	(A) The binding of SPN to importin-beta is increased upon mutation or truncation of the C terminus.	bind
8026	2	3248	5	11	NULL	0	NULL			mutation of	increases			C terminus		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4660_s_261	16030253	(A) The binding of SPN to importin-beta is increased upon mutation or truncation of the C terminus.	bind
8027	3	3248	5	11	NULL	0	NULL			truncation of	increases			C terminus		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4660_s_261	16030253	(A) The binding of SPN to importin-beta is increased upon mutation or truncation of the C terminus.	bind
8028	4	3248	5	11	NULL	0	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4660_s_261	16030253	(A) The binding of SPN to importin-beta is increased upon mutation or truncation of the C terminus.	bind
9976	1	3248	7	11	NULL	0	NULL	SPN	GP		bind					importin-beta	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4660_s_261	16030253	(A) The binding of SPN to importin-beta is increased upon mutation or truncation of the C terminus.	bind
9977	2	3248	7	11	NULL	0	NULL	statement 1	Process		is increased upon					C terminus	GP	mutation of			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4660_s_261	16030253	(A) The binding of SPN to importin-beta is increased upon mutation or truncation of the C terminus.	bind
9978	3	3248	7	11	NULL	0	NULL	statement 1	Process		is increased upon					C terminus	GP	truncation of			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4660_s_261	16030253	(A) The binding of SPN to importin-beta is increased upon mutation or truncation of the C terminus.	bind
12381	4	3248	7	11	NULL	0	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4660_s_261	16030253	(A) The binding of SPN to importin-beta is increased upon mutation or truncation of the C terminus.	bind
80176	1	3248	11	NULL	NULL	0	NULL	SPN	Protein		binds to 					importin-beta	Protein				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4660_s_261	16030253	(A) The binding of SPN to importin-beta is increased upon mutation or truncation of the C terminus.	bind
80177	2	3248	11	NULL	NULL	0	NULL	statement 1	Process		increased in					mutation	MolecularProcess	of the C terminus			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4660_s_261	16030253	(A) The binding of SPN to importin-beta is increased upon mutation or truncation of the C terminus.	bind
80178	3	3248	11	NULL	NULL	0	NULL	statement 1	Process		increased in					truncation	MolecularProcess	of the C terminus			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4660_s_261	16030253	(A) The binding of SPN to importin-beta is increased upon mutation or truncation of the C terminus.	bind
80179	4	3248	11	NULL	NULL	0	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4660_s_261	16030253	(A) The binding of SPN to importin-beta is increased upon mutation or truncation of the C terminus.	bind
8218	2	3249	5	11	NULL	0	NULL	tRNAIle	GP		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_4_4_519_s_52	10549284	(a) The binding of tRNAIle to IleRS complexed to a misactivated valine (Val ) first results in the translocation of the misactivated amino acid from the active site to the editing site (for this illustration, no distinction is made between misactivated valine as Val-AMP or as Val-tRNAIle).	bind
8219	1	3249	5	11	NULL	0	NULL	IleRS	GP		is in complex with					valine	AminoAcid	misactivated			NULL		NULL	NULL	NULL	NULL	gw60_molcell_4_4_519_s_52	10549284	(a) The binding of tRNAIle to IleRS complexed to a misactivated valine (Val ) first results in the translocation of the misactivated amino acid from the active site to the editing site (for this illustration, no distinction is made between misactivated valine as Val-AMP or as Val-tRNAIle).	bind
8220	3	3249	5	11	NULL	0	NULL	statement 2	Process		results in					amino acid	AminoAcid	translocation of;; misactivated 			NULL		NULL	NULL	NULL	NULL	gw60_molcell_4_4_519_s_52	10549284	(a) The binding of tRNAIle to IleRS complexed to a misactivated valine (Val ) first results in the translocation of the misactivated amino acid from the active site to the editing site (for this illustration, no distinction is made between misactivated valine as Val-AMP or as Val-tRNAIle).	bind
8221	4	3249	5	11	NULL	0	NULL	misactivated amino acid	AminoAcid		is translocated to					editing site	GP	from active site			NULL		NULL	NULL	NULL	NULL	gw60_molcell_4_4_519_s_52	10549284	(a) The binding of tRNAIle to IleRS complexed to a misactivated valine (Val ) first results in the translocation of the misactivated amino acid from the active site to the editing site (for this illustration, no distinction is made between misactivated valine as Val-AMP or as Val-tRNAIle).	bind
9979	2	3249	7	11	NULL	0	NULL	tRNAIle	GP		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_4_4_519_s_52	10549284	(a) The binding of tRNAIle to IleRS complexed to a misactivated valine (Val ) first results in the translocation of the misactivated amino acid from the active site to the editing site (for this illustration, no distinction is made between misactivated valine as Val-AMP or as Val-tRNAIle).	bind
9980	1	3249	7	11	NULL	0	NULL	IleRS	GP		is complexed to					valine 	AminoAcid	misactivated 			NULL		NULL	NULL	NULL	NULL	gw60_molcell_4_4_519_s_52	10549284	(a) The binding of tRNAIle to IleRS complexed to a misactivated valine (Val ) first results in the translocation of the misactivated amino acid from the active site to the editing site (for this illustration, no distinction is made between misactivated valine as Val-AMP or as Val-tRNAIle).	bind
9981	3	3249	7	11	NULL	0	NULL	statement 2	Process		results in 					amino acid	AminoAcid	misactivated;; translocation of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_4_4_519_s_52	10549284	(a) The binding of tRNAIle to IleRS complexed to a misactivated valine (Val ) first results in the translocation of the misactivated amino acid from the active site to the editing site (for this illustration, no distinction is made between misactivated valine as Val-AMP or as Val-tRNAIle).	bind
9982	4	3249	7	11	NULL	0	NULL	statement 3	Process		occurs from					editing site	GP	from the active site to			NULL		NULL	NULL	NULL	NULL	gw60_molcell_4_4_519_s_52	10549284	(a) The binding of tRNAIle to IleRS complexed to a misactivated valine (Val ) first results in the translocation of the misactivated amino acid from the active site to the editing site (for this illustration, no distinction is made between misactivated valine as Val-AMP or as Val-tRNAIle).	bind
9983	5	3249	7	11	NULL	0	NULL	valine	AminoAcid		is					Val	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_4_4_519_s_52	10549284	(a) The binding of tRNAIle to IleRS complexed to a misactivated valine (Val ) first results in the translocation of the misactivated amino acid from the active site to the editing site (for this illustration, no distinction is made between misactivated valine as Val-AMP or as Val-tRNAIle).	bind
80180	1	3249	11	NULL	NULL	0	NULL	 tRNAIle	NucleicAcidSubstance		binds to 					IleRS	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcell_4_4_519_s_52	10549284	(a) The binding of tRNAIle to IleRS complexed to a misactivated valine (Val ) first results in the translocation of the misactivated amino acid from the active site to the editing site (for this illustration, no distinction is made between misactivated valine as Val-AMP or as Val-tRNAIle).	bind
80181	2	3249	11	NULL	NULL	0	NULL	statement 1	NucleicAcidSubstance		complexed to					valine	AminoAcid	misactivated			NULL		0	NULL	NULL	NULL	gw60_molcell_4_4_519_s_52	10549284	(a) The binding of tRNAIle to IleRS complexed to a misactivated valine (Val ) first results in the translocation of the misactivated amino acid from the active site to the editing site (for this illustration, no distinction is made between misactivated valine as Val-AMP or as Val-tRNAIle).	bind
80182	3	3249	11	NULL	NULL	0	NULL	Val	AminoAcid		is					valine	AminoAcid				NULL		0	NULL	NULL	NULL	gw60_molcell_4_4_519_s_52	10549284	(a) The binding of tRNAIle to IleRS complexed to a misactivated valine (Val ) first results in the translocation of the misactivated amino acid from the active site to the editing site (for this illustration, no distinction is made between misactivated valine as Val-AMP or as Val-tRNAIle).	bind
80183	4	3249	11	NULL	NULL	NULL	NULL	valine	AminoAcid	misactivated;;from the active site	undergoes					translocation	MolecularProcess	to the editing site			NULL		NULL	NULL	NULL	NULL	gw60_molcell_4_4_519_s_52	10549284	(a) The binding of tRNAIle to IleRS complexed to a misactivated valine (Val ) first results in the translocation of the misactivated amino acid from the active site to the editing site (for this illustration, no distinction is made between misactivated valine as Val-AMP or as Val-tRNAIle).	bind
8029	1	3250	5	11	NULL	0	NULL	histone H3	GP	[35]methionine-labeled	bind					RbAP46	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_1_324_s_239	15601853	(A) The binding of [35]methionine-labeled histone H3 to RbAP46 was competed with hypo- or hyperacetylated  core histones.	bind
8030	2	3250	5	11	NULL	0	NULL	core histones	GP	hypoacetylated	bind					RbAP46	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_1_324_s_239	15601853	(A) The binding of [35]methionine-labeled histone H3 to RbAP46 was competed with hypo- or hyperacetylated  core histones.	bind
8031	3	3250	5	11	NULL	0	NULL	core histones	GP	hyperacetylated	bind					RbAP46	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_1_324_s_239	15601853	(A) The binding of [35]methionine-labeled histone H3 to RbAP46 was competed with hypo- or hyperacetylated  core histones.	bind
8032	4	3250	5	11	NULL	0	NULL	statement 2	GP		compete with					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_1_324_s_239	15601853	(A) The binding of [35]methionine-labeled histone H3 to RbAP46 was competed with hypo- or hyperacetylated  core histones.	bind
8033	5	3250	5	11	NULL	0	NULL	statement 3	GP		compete with					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_1_324_s_239	15601853	(A) The binding of [35]methionine-labeled histone H3 to RbAP46 was competed with hypo- or hyperacetylated  core histones.	bind
9984	1	3250	7	11	NULL	0	NULL	 histone H3	GP	[35]methionine-labeled	bind					RbAP46	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_1_324_s_239	15601853	(A) The binding of [35]methionine-labeled histone H3 to RbAP46 was competed with hypo- or hyperacetylated  core histones.	bind
9985	2	3250	7	11	NULL	0	NULL	 core histones	GP	hypoacetylated	bind					RbAP46	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_1_324_s_239	15601853	(A) The binding of [35]methionine-labeled histone H3 to RbAP46 was competed with hypo- or hyperacetylated  core histones.	bind
9986	3	3250	7	11	NULL	0	NULL	core histones	GP	hyperacetylated 	bind					RbAP46	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_1_324_s_239	15601853	(A) The binding of [35]methionine-labeled histone H3 to RbAP46 was competed with hypo- or hyperacetylated  core histones.	bind
9987	4	3250	7	11	NULL	0	NULL	statement 2	GP		compete with					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_1_324_s_239	15601853	(A) The binding of [35]methionine-labeled histone H3 to RbAP46 was competed with hypo- or hyperacetylated  core histones.	bind
9988	5	3250	7	11	NULL	0	NULL	statement 3	GP		compete with					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_1_324_s_239	15601853	(A) The binding of [35]methionine-labeled histone H3 to RbAP46 was competed with hypo- or hyperacetylated  core histones.	bind
80184	1	3250	11	NULL	NULL	0	NULL	histone H3	Protein	[35]methionine-labeled	binds to 					RbAP46	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_1_324_s_239	15601853	(A) The binding of [35]methionine-labeled histone H3 to RbAP46 was competed with hypo- or hyperacetylated  core histones.	bind
80185	2	3250	11	NULL	NULL	0	NULL	histones	Protein	hyperacetylated core	binds to 					RbAP46	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_1_324_s_239	15601853	(A) The binding of [35]methionine-labeled histone H3 to RbAP46 was competed with hypo- or hyperacetylated  core histones.	bind
80186	3	3250	11	NULL	NULL	0	NULL	histones	Protein	hypoacetylated core	binds to 					RbAP46	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_1_324_s_239	15601853	(A) The binding of [35]methionine-labeled histone H3 to RbAP46 was competed with hypo- or hyperacetylated  core histones.	bind
80187	4	3250	11	NULL	NULL	0	NULL	statement 1	Process		competes with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_1_324_s_239	15601853	(A) The binding of [35]methionine-labeled histone H3 to RbAP46 was competed with hypo- or hyperacetylated  core histones.	bind
80188	5	3250	11	NULL	NULL	0	NULL	statement 1	Process		competes with					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_1_324_s_239	15601853	(A) The binding of [35]methionine-labeled histone H3 to RbAP46 was competed with hypo- or hyperacetylated  core histones.	bind
8034	1	3251	5	11	NULL	0	NULL	CycT1	GP		bind			C-terminal region		CTD	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_1_321_s_206	11739744	(A) The C-terminal region of CycT1 binds the CTD in vitro.	bind
9989	1	3251	7	11	NULL	0	NULL	CycT1	GP		bind			C-terminal region		CTD	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_1_321_s_206	11739744	(A) The C-terminal region of CycT1 binds the CTD in vitro.	bind
80189	1	3251	11	NULL	NULL	0	NULL	CycT1	Gene	C-terminal 	binds to 								CTD		NULL	in vitro	0	NULL	NULL	NULL	gw60_molcellbiol_22_1_321_s_206	11739744	(A) The C-terminal region of CycT1 binds the CTD in vitro.	bind
8035	1	3252	5	11	NULL	0	NULL	C/EBPbeta	GP		bind				SBE in promoter	Stat1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2108_s_336	9528783	(A) The C/EBPbeta promoter contains an SBE that binds Stat1 and Stat3.	bind
8036	2	3252	5	11	NULL	0	NULL	C/EBPbeta	GP		bind				SBE in promoter	Stat3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2108_s_336	9528783	(A) The C/EBPbeta promoter contains an SBE that binds Stat1 and Stat3.	bind
9990	1	3252	7	11	NULL	0	NULL	Stat1	GP		bind					C/EBPbeta	GP			SBE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2108_s_336	9528783	(A) The C/EBPbeta promoter contains an SBE that binds Stat1 and Stat3.	bind
9991	2	3252	7	11	NULL	0	NULL	Stat3	GP		bind					C/EBPbeta	GP			SBE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2108_s_336	9528783	(A) The C/EBPbeta promoter contains an SBE that binds Stat1 and Stat3.	bind
80190	1	3252	11	NULL	NULL	0	NULL	C/EBPbeta promoter	NucleicAcidSubstance		contains					SBE	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_4_2108_s_336	9528783	(A) The C/EBPbeta promoter contains an SBE that binds Stat1 and Stat3.	bind
80191	2	3252	11	NULL	NULL	0	NULL	C/EBPbeta promoter	NucleicAcidSubstance		binds to 				SBE	Stat1	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_4_2108_s_336	9528783	(A) The C/EBPbeta promoter contains an SBE that binds Stat1 and Stat3.	bind
80192	3	3252	11	NULL	NULL	0	NULL	C/EBPbeta promoter	NucleicAcidSubstance		binds to 				SBE	Stat3	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_4_2108_s_336	9528783	(A) The C/EBPbeta promoter contains an SBE that binds Stat1 and Stat3.	bind
8037	1	3253	5	11	NULL	0	NULL	Adf-1	GP		bind			carboxy terminus		TAFII110	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2252_s_260	9528796	(A) The carboxy terminus of Adf-1 binds TAFII110 and TAFII250.	bind
8038	2	3253	5	11	NULL	0	NULL	Adf-1	GP		bind			carboxy terminus		TAFII250	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2252_s_260	9528796	(A) The carboxy terminus of Adf-1 binds TAFII110 and TAFII250.	bind
9992	1	3253	7	11	NULL	0	NULL	Adf-1	GP		bind			carboxy terminus		TAFII110	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2252_s_260	9528796	(A) The carboxy terminus of Adf-1 binds TAFII110 and TAFII250.	bind
9993	2	3253	7	11	NULL	0	NULL	Adf-1	GP		bind			carboxy terminus		TAFII250	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2252_s_260	9528796	(A) The carboxy terminus of Adf-1 binds TAFII110 and TAFII250.	bind
80193	1	3253	11	NULL	NULL	0	NULL	Adf-1	Protein	carboxy terminus	binds to 					TAFII110	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_4_2252_s_260	9528796	(A) The carboxy terminus of Adf-1 binds TAFII110 and TAFII250.	bind
80194	2	3253	11	NULL	NULL	0	NULL	Adf-1	Protein	carboxy terminus	binds to 					TAFII250	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_4_2252_s_260	9528796	(A) The carboxy terminus of Adf-1 binds TAFII110 and TAFII250.	bind
8039	1	3254	5	11	NULL	0	NULL	HDAC4	GP		bind			carboxyl-terminal region		PC4	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2242_s_444	15743821	(A) The carboxyl-terminal  region of HDAC4 binds PC4.	bind
9994	1	3254	7	11	NULL	0	NULL	HDAC4	GP		bind			carboxyl-terminal 		PC4	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2242_s_444	15743821	(A) The carboxyl-terminal  region of HDAC4 binds PC4.	bind
80195	1	3254	11	NULL	NULL	0	NULL	 HDAC4	Protein	carboxyl-terminal	binds to 					PC4	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_6_2242_s_444	15743821	(A) The carboxyl-terminal  region of HDAC4 binds PC4.	bind
8040	1	3255	5	11	NULL	NULL	NULL	CArG-like site	GP		bind		weakly		 - 122/ - 85 promoter fragment	SRF	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_131_3_669_s_76	14711876	(A) The CArG-like  site in  - 122/ - 85 promoter fragment binds SRF only weakly (complex labelled S);  GATA4 protein binds efficiently to the GATA#2 site present in the same probe (labelled  G); simultaneous binding of SRF and GATA4 can be detected (arrow).	bind
8041	2	3255	5	11	NULL	NULL	NULL	GATA4 protein	GP		bind		efficiently			probe	NucleicAcid			GATA#2 site	NULL		NULL	NULL	NULL	NULL	gw70_development_131_3_669_s_76	14711876	(A) The CArG-like  site in  - 122/ - 85 promoter fragment binds SRF only weakly (complex labelled S);  GATA4 protein binds efficiently to the GATA#2 site present in the same probe (labelled  G); simultaneous binding of SRF and GATA4 can be detected (arrow).	bind
8042	3	3255	5	11	NULL	0	NULL	statement 1	Process		occurs simultaneously with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_131_3_669_s_76	14711876	(A) The CArG-like  site in  - 122/ - 85 promoter fragment binds SRF only weakly (complex labelled S);  GATA4 protein binds efficiently to the GATA#2 site present in the same probe (labelled  G); simultaneous binding of SRF and GATA4 can be detected (arrow).	bind
10006	1	3255	7	11	NULL	0	NULL	CArG-like site	GP		bind		weakly		- 122/ - 85 promoter fragment	SRF	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_131_3_669_s_76	14711876	(A) The CArG-like  site in  - 122/ - 85 promoter fragment binds SRF only weakly (complex labelled S);  GATA4 protein binds efficiently to the GATA#2 site present in the same probe (labelled  G); simultaneous binding of SRF and GATA4 can be detected (arrow).	bind
10007	2	3255	7	11	NULL	0	NULL	GATA4	GP		bind		efficiently							GATA#2 site	NULL		NULL	NULL	NULL	NULL	gw70_development_131_3_669_s_76	14711876	(A) The CArG-like  site in  - 122/ - 85 promoter fragment binds SRF only weakly (complex labelled S);  GATA4 protein binds efficiently to the GATA#2 site present in the same probe (labelled  G); simultaneous binding of SRF and GATA4 can be detected (arrow).	bind
10008	3	3255	7	11	NULL	0	NULL	statement 1	Process		occur simultaneously with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_131_3_669_s_76	14711876	(A) The CArG-like  site in  - 122/ - 85 promoter fragment binds SRF only weakly (complex labelled S);  GATA4 protein binds efficiently to the GATA#2 site present in the same probe (labelled  G); simultaneous binding of SRF and GATA4 can be detected (arrow).	bind
81258	1	3255	11	NULL	NULL	0	NULL	SRF	GeneOrProtein		binds to 		simultaneously			GATA4	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw70_development_131_3_669_s_76	14711876	(A) The CArG-like  site in  - 122/ - 85 promoter fragment binds SRF only weakly (complex labelled S);  GATA4 protein binds efficiently to the GATA#2 site present in the same probe (labelled  G); simultaneous binding of SRF and GATA4 can be detected (arrow).	bind
80196	1	3256	11	NULL	NULL	0	NULL	FOXO	Protein		is a type of 					Forkhead transcription factor	Protein				NULL		0	NULL	NULL	NULL	gw70_cellbiol_162_4_613_s_137	12913110	(A) The consensus binding site for the FOXO subfamily of Forkhead transcription factors  and a known FOXO binding site in the Fas ligand promoter (FasL) are compared with  the conserved bim1 and bim2 sites located close to the  bim promoter.	bind
80197	2	3256	11	NULL	NULL	0	NULL	FasL	Protein		is					Fas ligand promoter	Protein				NULL		0	NULL	NULL	NULL	gw70_cellbiol_162_4_613_s_137	12913110	(A) The consensus binding site for the FOXO subfamily of Forkhead transcription factors  and a known FOXO binding site in the Fas ligand promoter (FasL) are compared with  the conserved bim1 and bim2 sites located close to the  bim promoter.	bind
80198	3	3256	11	NULL	NULL	0	NULL	bim1	NucleicAcidSubstance	conserved sites	located close to					bim promoter	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_cellbiol_162_4_613_s_137	12913110	(A) The consensus binding site for the FOXO subfamily of Forkhead transcription factors  and a known FOXO binding site in the Fas ligand promoter (FasL) are compared with  the conserved bim1 and bim2 sites located close to the  bim promoter.	bind
80199	4	3256	11	NULL	NULL	0	NULL	bim2	NucleicAcidSubstance	conserved sites	located close to					bim promoter	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_cellbiol_162_4_613_s_137	12913110	(A) The consensus binding site for the FOXO subfamily of Forkhead transcription factors  and a known FOXO binding site in the Fas ligand promoter (FasL) are compared with  the conserved bim1 and bim2 sites located close to the  bim promoter.	bind
8043	1	3257	5	11	NULL	0	NULL	[125]GA3	GP		bind					SMMC7721-Tie2	Cell				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_315_4_1004_s_84	14985112	(A) The counts of [125]GA3 bound to Tie2 positive expressing SMMC7721-Tie2 and Tie2 negative parent cells  SMMC7721 with (GA3*/GA3) or without (GA3*) addition of 100-fold molar excess of cold  GA3.	bind
8044	2	3257	5	11	NULL	0	NULL	[125]GA3	GP		bind					SMMC7721	Cell				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_315_4_1004_s_84	14985112	(A) The counts of [125]GA3 bound to Tie2 positive expressing SMMC7721-Tie2 and Tie2 negative parent cells  SMMC7721 with (GA3*/GA3) or without (GA3*) addition of 100-fold molar excess of cold  GA3.	bind
44753	3	3257	5	11	NULL	0	NULL	SMMC7721-Tie2	Cell		is a type of					Tie2 positive expressing cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_315_4_1004_s_84	14985112	(A) The counts of [125]GA3 bound to Tie2 positive expressing SMMC7721-Tie2 and Tie2 negative parent cells  SMMC7721 with (GA3*/GA3) or without (GA3*) addition of 100-fold molar excess of cold  GA3.	bind
44754	4	3257	5	11	NULL	0	NULL	SMMC7721	Cell		is a type of					Tie2 negative parent cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_315_4_1004_s_84	14985112	(A) The counts of [125]GA3 bound to Tie2 positive expressing SMMC7721-Tie2 and Tie2 negative parent cells  SMMC7721 with (GA3*/GA3) or without (GA3*) addition of 100-fold molar excess of cold  GA3.	bind
10084	1	3257	7	11	NULL	0	NULL	[125]GA3	GP		bind					SMMC7721-Tie2 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_315_4_1004_s_84	14985112	(A) The counts of [125]GA3 bound to Tie2 positive expressing SMMC7721-Tie2 and Tie2 negative parent cells  SMMC7721 with (GA3*/GA3) or without (GA3*) addition of 100-fold molar excess of cold  GA3.	bind
10085	2	3257	7	11	NULL	0	NULL	[125]GA3	GP		bind					SMMC7721 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_315_4_1004_s_84	14985112	(A) The counts of [125]GA3 bound to Tie2 positive expressing SMMC7721-Tie2 and Tie2 negative parent cells  SMMC7721 with (GA3*/GA3) or without (GA3*) addition of 100-fold molar excess of cold  GA3.	bind
44755	3	3257	7	11	NULL	0	NULL	SMMC7721-Tie2	Cell		is a type of					Tie2 positive expressing cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_315_4_1004_s_84	14985112	(A) The counts of [125]GA3 bound to Tie2 positive expressing SMMC7721-Tie2 and Tie2 negative parent cells  SMMC7721 with (GA3*/GA3) or without (GA3*) addition of 100-fold molar excess of cold  GA3.	bind
44756	4	3257	7	11	NULL	0	NULL	SMMC7721	Cell		is a type of					Tie2 negative parent cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_315_4_1004_s_84	14985112	(A) The counts of [125]GA3 bound to Tie2 positive expressing SMMC7721-Tie2 and Tie2 negative parent cells  SMMC7721 with (GA3*/GA3) or without (GA3*) addition of 100-fold molar excess of cold  GA3.	bind
8045	1	3258	5	11	NULL	0	NULL	L11	NucleicAcid		bind								L11BD		NULL		NULL	NULL	NULL	NULL	gw60_chembiol_10_8_769_s_143	12954336	(A) The crystal structure of L11 bound to L11BD  [24]   is overlaid onto the L11BD coordinates.	bind
10009	1	3258	7	11	NULL	0	NULL	L11 	NucleicAcid		bind					 			L11BD		NULL		NULL	NULL	NULL	NULL	gw60_chembiol_10_8_769_s_143	12954336	(A) The crystal structure of L11 bound to L11BD  [24]   is overlaid onto the L11BD coordinates.	bind
80200	1	3258	11	NULL	NULL	0	NULL	L11	Protein		binds to 								L11BD		NULL		0	NULL	NULL	NULL	gw60_chembiol_10_8_769_s_143	12954336	(A) The crystal structure of L11 bound to L11BD  [24]   is overlaid onto the L11BD coordinates.	bind
8046	1	3259	5	11	NULL	0	NULL	pRB	GP		bind					E7 peptide	GP	papillomavirus			NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_2_179_s_102	12040123	(A) The crystal structure of pRB  bound to an E7 peptide (from papillomavirus) containing an LXCXE motif (PDB code  1Gux [ ]).	bind
8047	2	3259	5	11	NULL	0	NULL	E7 peptide	GP	papillomavirus	contain								LXCXE motif		NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_2_179_s_102	12040123	(A) The crystal structure of pRB  bound to an E7 peptide (from papillomavirus) containing an LXCXE motif (PDB code  1Gux [ ]).	bind
10010	1	3259	7	11	NULL	0	NULL	 pRB	GP		bind					E7 peptide	GP	papillomavirus			NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_2_179_s_102	12040123	(A) The crystal structure of pRB  bound to an E7 peptide (from papillomavirus) containing an LXCXE motif (PDB code  1Gux [ ]).	bind
12386	2	3259	7	11	NULL	0	NULL	E7 peptide	GP		contain								LXCXE motif		NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_2_179_s_102	12040123	(A) The crystal structure of pRB  bound to an E7 peptide (from papillomavirus) containing an LXCXE motif (PDB code  1Gux [ ]).	bind
80201	1	3259	11	NULL	NULL	0	NULL	pRB	Protein	crystal structure	binds to 					E7 peptide	PartOfProtein	papillomavirus	LXCXE motif		NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_2_179_s_102	12040123	(A) The crystal structure of pRB  bound to an E7 peptide (from papillomavirus) containing an LXCXE motif (PDB code  1Gux [ ]).	bind
8048	1	3261	5	11	NULL	0	NULL	cortactin protein	GP		contain								F-actin-binding sites		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_6_2162_s_90	12612086	(a) The diagram depicts different domains of the cortactin protein including the F-actin-binding sites, C-terminal tyrosines that are phosphorylated by Src kinases, and the SH3 domain that binds Dyn2.	bind
8049	2	3261	5	11	NULL	0	NULL	Src kinases	GP		phosphorylate					cortactin protein	GP		C-terminal tyrosines		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_6_2162_s_90	12612086	(a) The diagram depicts different domains of the cortactin protein including the F-actin-binding sites, C-terminal tyrosines that are phosphorylated by Src kinases, and the SH3 domain that binds Dyn2.	bind
8050	3	3261	5	11	NULL	0	NULL	cortactin protein	GP		bind			SH3 domain		Dyn2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_6_2162_s_90	12612086	(a) The diagram depicts different domains of the cortactin protein including the F-actin-binding sites, C-terminal tyrosines that are phosphorylated by Src kinases, and the SH3 domain that binds Dyn2.	bind
10011	1	3261	7	11	NULL	0	NULL	cortactin	GP		bind			SH3		Dyn2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_6_2162_s_90	12612086	(a) The diagram depicts different domains of the cortactin protein including the F-actin-binding sites, C-terminal tyrosines that are phosphorylated by Src kinases, and the SH3 domain that binds Dyn2.	bind
10012	2	3261	7	11	NULL	0	NULL	cortactin	GP		phosphorylated by			C-terminal tyrosines		Src kinases	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_6_2162_s_90	12612086	(a) The diagram depicts different domains of the cortactin protein including the F-actin-binding sites, C-terminal tyrosines that are phosphorylated by Src kinases, and the SH3 domain that binds Dyn2.	bind
10013	3	3261	7	11	NULL	0	NULL	cortactin	GP		has					 F-actin-binding site	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_6_2162_s_90	12612086	(a) The diagram depicts different domains of the cortactin protein including the F-actin-binding sites, C-terminal tyrosines that are phosphorylated by Src kinases, and the SH3 domain that binds Dyn2.	bind
80202	1	3261	11	NULL	NULL	0	NULL	cortactin protein	Protein		binds to 			SH3 domain		Dyn2	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_6_2162_s_90	12612086	(a) The diagram depicts different domains of the cortactin protein including the F-actin-binding sites, C-terminal tyrosines that are phosphorylated by Src kinases, and the SH3 domain that binds Dyn2.	bind
80203	2	3261	11	NULL	NULL	0	NULL	 Src kinase	Protein		phosphorylate					cortactin protein			C-terminal tyrosines		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_6_2162_s_90	12612086	(a) The diagram depicts different domains of the cortactin protein including the F-actin-binding sites, C-terminal tyrosines that are phosphorylated by Src kinases, and the SH3 domain that binds Dyn2.	bind
80204	3	3261	11	NULL	NULL	0	NULL	cortactin protein	Protein		has binding site for					 F-actin					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_6_2162_s_90	12612086	(a) The diagram depicts different domains of the cortactin protein including the F-actin-binding sites, C-terminal tyrosines that are phosphorylated by Src kinases, and the SH3 domain that binds Dyn2.	bind
8053	1	3262	5	11	NULL	0	NULL	FBP17	GP		bind		strongly	EFC domain		PS	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_172_2_269_s_85	16418535	(A) The EFC domain of FBP17 strongly bound to PS and PI(4,5)P2.	bind
8054	2	3262	5	11	NULL	0	NULL	FBP17	GP		bind		strongly	EFC domain		PI(4,5)P2	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_172_2_269_s_85	16418535	(A) The EFC domain of FBP17 strongly bound to PS and PI(4,5)P2.	bind
10014	1	3262	7	11	NULL	0	NULL	FBP17 	GP		bind		strongly	EFC		PS	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_172_2_269_s_85	16418535	(A) The EFC domain of FBP17 strongly bound to PS and PI(4,5)P2.	bind
10015	2	3262	7	11	NULL	0	NULL	FBP17	GP		bind		strongly	EFC		PI(4,5)P2	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_172_2_269_s_85	16418535	(A) The EFC domain of FBP17 strongly bound to PS and PI(4,5)P2.	bind
80205	1	3262	11	NULL	NULL	0	NULL	FBP17	Protein		binds to 			EFC domain		PS	Protein				NULL		0	NULL	NULL	NULL	gw70_cellbiol_172_2_269_s_85	16418535	(A) The EFC domain of FBP17 strongly bound to PS and PI(4,5)P2.	bind
80206	2	3262	11	NULL	NULL	0	NULL	FBP17	Protein		binds to 			EFC domain		PI(4,5)P2	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	gw70_cellbiol_172_2_269_s_85	16418535	(A) The EFC domain of FBP17 strongly bound to PS and PI(4,5)P2.	bind
8055	1	3264	5	11	NULL	0	NULL	ANS	Chemical		bind		efficiently			EF-Ts	GP	thermally denatured form of			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1764_7_1277_s_35	16781902	(A) The emission spectra of thermally denatured EF-Ts(wt) with ANS (EF-Ts + ANS(T))  and native EF-Ts(wt) with ANS (EF-Ts + ANS) show efficient binding of ANS into thermally  denatured form of EF-Ts.	bind
10016	1	3264	7	11	NULL	0	NULL	EF-Ts	GP	thermally denatured wt	bind		efficiently			ANS	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1764_7_1277_s_35	16781902	(A) The emission spectra of thermally denatured EF-Ts(wt) with ANS (EF-Ts + ANS(T))  and native EF-Ts(wt) with ANS (EF-Ts + ANS) show efficient binding of ANS into thermally  denatured form of EF-Ts.	bind
80207	1	3264	11	NULL	NULL	0	NULL	ANS	Chemical		binds to 					EF-Ts	Protein	thermally denatured 			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1764_7_1277_s_35	16781902	(A) The emission spectra of thermally denatured EF-Ts(wt) with ANS (EF-Ts + ANS(T))  and native EF-Ts(wt) with ANS (EF-Ts + ANS) show efficient binding of ANS into thermally  denatured form of EF-Ts.	bind
8056	1	3265	5	11	NULL	0	NULL	MutL proteins	GP	mutant 	bind		equilibrium			ATP S	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_233_s_228	12887908	(A) The equilibrium binding of ATP S by MutL mutant proteins.	bind
10020	1	3265	7	11	NULL	0	NULL	ATP S	Chemical		bind		equilibrium			MutL	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_233_s_228	12887908	(A) The equilibrium binding of ATP S by MutL mutant proteins.	bind
80208	1	3265	11	NULL	NULL	0	NULL	MutL protein	Protein	mutant	binds to 					ATP S	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcell_12_1_233_s_228	12887908	(A) The equilibrium binding of ATP S by MutL mutant proteins.	bind
10042	1	3269	5	11	NULL	0	NULL	Npn-1	GP	deletion mutant	is expressed in					COS7 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_5_1093_s_65	9856464	(A) The indicated deletion mutants of Npn-1 were expressed in COS7 cells, and binding of the full length c-semD (10 nM c-semD-AP), the sema domain ligand (10 nM CAP-4), or the basic-rich carboxyl tail ligand (10 nM basic) was visualized by staining for bound AP.	bind
10043	2	3269	5	11	NULL	0	NULL	statement 1	Cell		bind					c-semD	Chemical	full length			NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_5_1093_s_65	9856464	(A) The indicated deletion mutants of Npn-1 were expressed in COS7 cells, and binding of the full length c-semD (10 nM c-semD-AP), the sema domain ligand (10 nM CAP-4), or the basic-rich carboxyl tail ligand (10 nM basic) was visualized by staining for bound AP.	bind
10044	3	3269	5	11	NULL	0	NULL	statement 1	Cell		bind					CAP-4	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_5_1093_s_65	9856464	(A) The indicated deletion mutants of Npn-1 were expressed in COS7 cells, and binding of the full length c-semD (10 nM c-semD-AP), the sema domain ligand (10 nM CAP-4), or the basic-rich carboxyl tail ligand (10 nM basic) was visualized by staining for bound AP.	bind
10045	4	3269	5	11	NULL	0	NULL	statement 1	Cell		bind					ligand	Chemical	basic-rich	carboxyl tail		NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_5_1093_s_65	9856464	(A) The indicated deletion mutants of Npn-1 were expressed in COS7 cells, and binding of the full length c-semD (10 nM c-semD-AP), the sema domain ligand (10 nM CAP-4), or the basic-rich carboxyl tail ligand (10 nM basic) was visualized by staining for bound AP.	bind
54240	5	3269	5	11	NULL	0	NULL	CAP-4	Chemical		is a type of					sema domain ligand	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_5_1093_s_65	9856464	(A) The indicated deletion mutants of Npn-1 were expressed in COS7 cells, and binding of the full length c-semD (10 nM c-semD-AP), the sema domain ligand (10 nM CAP-4), or the basic-rich carboxyl tail ligand (10 nM basic) was visualized by staining for bound AP.	bind
10021	1	3269	7	11	NULL	0	NULL	c-semD	Chemical		bind					AP					NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_5_1093_s_65	9856464	(A) The indicated deletion mutants of Npn-1 were expressed in COS7 cells, and binding of the full length c-semD (10 nM c-semD-AP), the sema domain ligand (10 nM CAP-4), or the basic-rich carboxyl tail ligand (10 nM basic) was visualized by staining for bound AP.	bind
10022	2	3269	7	11	NULL	0	NULL	sema domain ligand	Chemical		bind					AP					NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_5_1093_s_65	9856464	(A) The indicated deletion mutants of Npn-1 were expressed in COS7 cells, and binding of the full length c-semD (10 nM c-semD-AP), the sema domain ligand (10 nM CAP-4), or the basic-rich carboxyl tail ligand (10 nM basic) was visualized by staining for bound AP.	bind
10023	3	3269	7	11	NULL	0	NULL	basic-rich carboxyl tail ligand	Chemical		bind					AP					NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_5_1093_s_65	9856464	(A) The indicated deletion mutants of Npn-1 were expressed in COS7 cells, and binding of the full length c-semD (10 nM c-semD-AP), the sema domain ligand (10 nM CAP-4), or the basic-rich carboxyl tail ligand (10 nM basic) was visualized by staining for bound AP.	bind
80209	1	3269	11	NULL	NULL	0	NULL	Npn-1	Protein	deletion mutants	were expressed in					COS7 cells	Cell				NULL		0	NULL	NULL	NULL	gw60_neuron_21_5_1093_s_65	9856464	(A) The indicated deletion mutants of Npn-1 were expressed in COS7 cells, and binding of the full length c-semD (10 nM c-semD-AP), the sema domain ligand (10 nM CAP-4), or the basic-rich carboxyl tail ligand (10 nM basic) was visualized by staining for bound AP.	bind
80210	2	3269	11	NULL	NULL	0	NULL	statement 1	Protein		binds to 					c-semD	Protein				NULL		0	NULL	NULL	NULL	gw60_neuron_21_5_1093_s_65	9856464	(A) The indicated deletion mutants of Npn-1 were expressed in COS7 cells, and binding of the full length c-semD (10 nM c-semD-AP), the sema domain ligand (10 nM CAP-4), or the basic-rich carboxyl tail ligand (10 nM basic) was visualized by staining for bound AP.	bind
80211	3	3269	11	NULL	NULL	0	NULL	CAP-4	Protein		is a type of 					sema domain ligand	Protein				NULL		0	NULL	NULL	NULL	gw60_neuron_21_5_1093_s_65	9856464	(A) The indicated deletion mutants of Npn-1 were expressed in COS7 cells, and binding of the full length c-semD (10 nM c-semD-AP), the sema domain ligand (10 nM CAP-4), or the basic-rich carboxyl tail ligand (10 nM basic) was visualized by staining for bound AP.	bind
80212	4	3269	11	NULL	NULL	0	NULL	Npn-1	Protein	deletion mutants	binds to 					sema domain ligand	Protein				NULL		0	NULL	NULL	NULL	gw60_neuron_21_5_1093_s_65	9856464	(A) The indicated deletion mutants of Npn-1 were expressed in COS7 cells, and binding of the full length c-semD (10 nM c-semD-AP), the sema domain ligand (10 nM CAP-4), or the basic-rich carboxyl tail ligand (10 nM basic) was visualized by staining for bound AP.	bind
80213	5	3269	11	NULL	NULL	0	NULL	Npn-1	Protein	deletion mutants	binds to 					basic-rich carboxyl tail ligand	Protein				NULL		0	NULL	NULL	NULL	gw60_neuron_21_5_1093_s_65	9856464	(A) The indicated deletion mutants of Npn-1 were expressed in COS7 cells, and binding of the full length c-semD (10 nM c-semD-AP), the sema domain ligand (10 nM CAP-4), or the basic-rich carboxyl tail ligand (10 nM basic) was visualized by staining for bound AP.	bind
8058	1	3270	5	11	NULL	0	NULL	migfilin	GP		bind					filamin	GP		C-terminal fragment		NULL		NULL	NULL	NULL	NULL	gw60_cell_113_1_37_s_192	12679033	(A) The interaction between migfilin and filamin C-terminal fragments containing different repeats were determined by yeast two-hybrid binding assays as described in the Experimental Procedures.	bind
10026	1	3270	7	11	NULL	0	NULL	migfilin	GP		bind					filamin	GP		C-terminal fragment		NULL		NULL	NULL	NULL	NULL	gw60_cell_113_1_37_s_192	12679033	(A) The interaction between migfilin and filamin C-terminal fragments containing different repeats were determined by yeast two-hybrid binding assays as described in the Experimental Procedures.	bind
80214	1	3270	11	NULL	NULL	0	NULL	migfilin	PartOfProtein	C-terminal fragments	interact with					filamin	PartOfProtein	C-terminal fragments			NULL		0	NULL	NULL	NULL	gw60_cell_113_1_37_s_192	12679033	(A) The interaction between migfilin and filamin C-terminal fragments containing different repeats were determined by yeast two-hybrid binding assays as described in the Experimental Procedures.	bind
80215	2	3270	11	NULL	NULL	0	NULL	statement 1	Process		determined by					yeast two-hybrid binding assays	ResearchActivity				NULL		0	NULL	NULL	NULL	gw60_cell_113_1_37_s_192	12679033	(A) The interaction between migfilin and filamin C-terminal fragments containing different repeats were determined by yeast two-hybrid binding assays as described in the Experimental Procedures.	bind
8059	1	3271	5	11	NULL	0	NULL	CD27	GP	intracellular region of 	does not bind					Ku	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_immunity_11_3_339_s_78	10514012	(A) The intracellular region of CD27 or that of CD30 does not bind to Ku.	bind
8060	2	3271	5	11	NULL	0	NULL	CD30	GP	intracellular region of	does not bind					Ku	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_immunity_11_3_339_s_78	10514012	(A) The intracellular region of CD27 or that of CD30 does not bind to Ku.	bind
10027	1	3271	7	11	NULL	0	NULL	CD27	GP	intracellular region of	does not bind					Ku	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_immunity_11_3_339_s_78	10514012	(A) The intracellular region of CD27 or that of CD30 does not bind to Ku.	bind
10028	2	3271	7	11	NULL	0	NULL	CD30	GP	intracellular region of	does not bind					Ku	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_immunity_11_3_339_s_78	10514012	(A) The intracellular region of CD27 or that of CD30 does not bind to Ku.	bind
80216	1	3271	11	NULL	NULL	0	NULL	CD27	Protein	intracellular region	does not bind to					Ku	Protein				NULL		0	NULL	NULL	NULL	gw60_immunity_11_3_339_s_78	10514012	(A) The intracellular region of CD27 or that of CD30 does not bind to Ku.	bind
80217	2	3271	11	NULL	NULL	0	NULL	CD30	Protein	intracellular region	does not bind to					Ku	Protein				NULL		0	NULL	NULL	NULL	gw60_immunity_11_3_339_s_78	10514012	(A) The intracellular region of CD27 or that of CD30 does not bind to Ku.	bind
8061	1	3272	5	11	NULL	0	NULL	AtMYB2	GP		bind					MBS-1 sequence	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genetics_149_2_479_s_123	9611167	(A) The left panel shows binding of AtMYB2 to both MBS-1 and MBS-2 sequences.	bind
8062	2	3272	5	11	NULL	0	NULL	AtMYB2	GP		bind					MBS-2 sequence	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genetics_149_2_479_s_123	9611167	(A) The left panel shows binding of AtMYB2 to both MBS-1 and MBS-2 sequences.	bind
10033	1	3272	7	11	NULL	0	NULL	AtMYB2	GP		bind					MBS-1 sequence	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genetics_149_2_479_s_123	9611167	(A) The left panel shows binding of AtMYB2 to both MBS-1 and MBS-2 sequences.	bind
10034	2	3272	7	11	NULL	0	NULL	AtMYB2	GP		bind					MBS-2 sequence	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genetics_149_2_479_s_123	9611167	(A) The left panel shows binding of AtMYB2 to both MBS-1 and MBS-2 sequences.	bind
80218	1	3272	11	NULL	NULL	0	NULL	AtMYB2	Protein		binds to 					MBS-1 sequences	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_genetics_149_2_479_s_123	9611167	(A) The left panel shows binding of AtMYB2 to both MBS-1 and MBS-2 sequences.	bind
80219	2	3272	11	NULL	NULL	0	NULL	AtMYB2	Protein		binds to 					MBS-2 sequence	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_genetics_149_2_479_s_123	9611167	(A) The left panel shows binding of AtMYB2 to both MBS-1 and MBS-2 sequences.	bind
80220	1	3274	11	NULL	NULL	0	NULL	FGFR1-IIIc	Protein	ligand binding regions	fused to					immunoglobulin 	Protein	 mouse	Fc fragment		NULL		0	NULL	NULL	NULL	gw70_development_131_14_3333_s_101	15201222	(A) The ligand binding regions of FGFR1-IIIc and FGFR2-IIIb (red) were fused to the  Fc fragment of a mouse immunoglobulin (blue) to generated secreted receptor versions.	bind
80221	2	3274	11	NULL	NULL	0	NULL	FGFR2-IIIb	Protein		fused to					immunoglobulin	Protein	mouse\t	Fc fragment		NULL		0	NULL	NULL	NULL	gw70_development_131_14_3333_s_101	15201222	(A) The ligand binding regions of FGFR1-IIIc and FGFR2-IIIb (red) were fused to the  Fc fragment of a mouse immunoglobulin (blue) to generated secreted receptor versions.	bind
8064	1	3275	5	11	NULL	0	NULL	ATP S	Chemical		bind					MutL	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_233_s_253	12887908	(A) The MutH protein enhanced ATP S binding by MutL.	bind
8065	2	3275	5	11	NULL	0	NULL	MutH protein	GP		enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_233_s_253	12887908	(A) The MutH protein enhanced ATP S binding by MutL.	bind
10036	1	3275	7	11	NULL	0	NULL	ATP S	Chemical		bind					MutL	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_233_s_253	12887908	(A) The MutH protein enhanced ATP S binding by MutL.	bind
10037	2	3275	7	11	NULL	0	NULL	MutH	GP		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_233_s_253	12887908	(A) The MutH protein enhanced ATP S binding by MutL.	bind
80222	1	3275	11	NULL	NULL	0	NULL	MutL	Protein		binds to 					ATP S	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcell_12_1_233_s_253	12887908	(A) The MutH protein enhanced ATP S binding by MutL.	bind
80223	2	3275	11	NULL	NULL	0	NULL	MutH protein	Protein		enhances					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_12_1_233_s_253	12887908	(A) The MutH protein enhanced ATP S binding by MutL.	bind
8063	1	3276	5	11	NULL	0	NULL	MutS protein	GP		bind					G/T mismatch DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_233_s_174	12887908	(A) The MutS protein (200 nM) was bound to G/T mismatch DNA in buffer B (marked  MutS ).	bind
10038	1	3276	7	11	NULL	0	NULL	MutS protein	GP		bind					G/T mismatch DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_233_s_174	12887908	(A) The MutS protein (200 nM) was bound to G/T mismatch DNA in buffer B (marked  MutS ).	bind
80224	1	3276	11	NULL	NULL	0	NULL	MutS protein	Protein		binds to 					DNA	NucleicAcidSubstance	in buffer B		G/T mismatch	NULL		0	NULL	NULL	NULL	gw60_molcell_12_1_233_s_174	12887908	(A) The MutS protein (200 nM) was bound to G/T mismatch DNA in buffer B (marked  MutS ).	bind
8066	1	3277	5	11	NULL	0	NULL	CNN	GP		bind			NH2-terminal domain		gamma-tubulin	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_162_5_757_s_60	12939255	(A) The NH2-terminal domain of CNN binds to gamma-tubulin.	bind
10039	1	3277	7	11	NULL	0	NULL	CNN	GP		bind			NH2-terminal domain		gamma-tubulin	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_162_5_757_s_60	12939255	(A) The NH2-terminal domain of CNN binds to gamma-tubulin.	bind
80225	1	3277	11	NULL	NULL	0	NULL	CNN	Protein		binds to 			NH2-terminal domain		gamma-tubulin	Protein				NULL		0	NULL	NULL	NULL	gw70_cellbiol_162_5_757_s_60	12939255	(A) The NH2-terminal domain of CNN binds to gamma-tubulin.	bind
8067	1	3278	5	11	NULL	0	NULL	NXF3 protein	GP		bind		specifically			Crm1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_2_397_s_109	11545741	(A) The NXF3 protein binds Crm1 specifically in a mammalian two-hybrid assay.	bind
10040	1	3278	7	11	NULL	0	NULL	NXF3	GP		bind		specifically			Crm1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_2_397_s_109	11545741	(A) The NXF3 protein binds Crm1 specifically in a mammalian two-hybrid assay.	bind
80226	1	3278	11	NULL	NULL	0	NULL	 NXF3 protein	Protein		binds to 					Crm1	Protein				NULL	mammalian two-hybrid assay	0	NULL	NULL	NULL	gw60_molcell_8_2_397_s_109	11545741	(A) The NXF3 protein binds Crm1 specifically in a mammalian two-hybrid assay.	bind
8068	1	3279	5	11	NULL	0	NULL	H5 peptide	GP		bind					SDS micelle	Chemical				NULL	in solution	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1545_1_153_s_117	11342041	(a) The overall structures of the H5 peptide bound to SDS micelle in solution, shown as a superposition of the backbone heavy atoms of the ten lowest energy structures, obtained by distance geometry and simulated annealing calculations.	bind
10041	1	3279	7	11	NULL	0	NULL	H5 peptide	GP		bind					SDS micelle	Chemical				NULL	in solution	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1545_1_153_s_117	11342041	(a) The overall structures of the H5 peptide bound to SDS micelle in solution, shown as a superposition of the backbone heavy atoms of the ten lowest energy structures, obtained by distance geometry and simulated annealing calculations.	bind
80227	1	3279	11	NULL	NULL	0	NULL	H5 peptide	PartOfProtein		binds to 					SDS micelle	Chemical				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1545_1_153_s_117	11342041	(a) The overall structures of the H5 peptide bound to SDS micelle in solution, shown as a superposition of the backbone heavy atoms of the ten lowest energy structures, obtained by distance geometry and simulated annealing calculations.	bind
80228	1	3280	11	NULL	NULL	0	NULL	PAX3-FKHR chimeric transcription factor	Protein		generated by					t(2;13) translocation	MolecularProcess	 in alveolar rhabdomyosarcoma			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_14_5019_s_31	10866659	(A) The PAX3-FKHR chimeric transcription factor generated by the t(2;13) translocation in alveolar rhabdomyosarcoma (ARMS) retains the PAX3 paired box (PB) and homeodomain (HD) DNA binding motifs, has a disrupted forkhead (FD) DNA binding domain, and acquires a COOH-terminal FKHR-derived activation domain.	bind
80229	2	3280	11	NULL	NULL	0	NULL	alveolar rhabdomyosarcoma	Disease		is					ARMS	Disease				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_14_5019_s_31	10866659	(A) The PAX3-FKHR chimeric transcription factor generated by the t(2;13) translocation in alveolar rhabdomyosarcoma (ARMS) retains the PAX3 paired box (PB) and homeodomain (HD) DNA binding motifs, has a disrupted forkhead (FD) DNA binding domain, and acquires a COOH-terminal FKHR-derived activation domain.	bind
80230	3	3280	11	NULL	NULL	0	NULL	PAX3-FKHR chimeric transcription factor	Protein		retains					PAX3 paired box	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_14_5019_s_31	10866659	(A) The PAX3-FKHR chimeric transcription factor generated by the t(2;13) translocation in alveolar rhabdomyosarcoma (ARMS) retains the PAX3 paired box (PB) and homeodomain (HD) DNA binding motifs, has a disrupted forkhead (FD) DNA binding domain, and acquires a COOH-terminal FKHR-derived activation domain.	bind
80231	4	3280	11	NULL	NULL	0	NULL	PAX3-FKHR chimeric transcription factor	Protein		retains								homeodomain		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_14_5019_s_31	10866659	(A) The PAX3-FKHR chimeric transcription factor generated by the t(2;13) translocation in alveolar rhabdomyosarcoma (ARMS) retains the PAX3 paired box (PB) and homeodomain (HD) DNA binding motifs, has a disrupted forkhead (FD) DNA binding domain, and acquires a COOH-terminal FKHR-derived activation domain.	bind
80232	5	3280	11	NULL	NULL	0	NULL	PAX3 paired box	Protein		is					PB	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_14_5019_s_31	10866659	(A) The PAX3-FKHR chimeric transcription factor generated by the t(2;13) translocation in alveolar rhabdomyosarcoma (ARMS) retains the PAX3 paired box (PB) and homeodomain (HD) DNA binding motifs, has a disrupted forkhead (FD) DNA binding domain, and acquires a COOH-terminal FKHR-derived activation domain.	bind
80233	6	3280	11	NULL	NULL	0	NULL	homeodomain	PartOfProtein		is					HD	PartOfProtein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_14_5019_s_31	10866659	(A) The PAX3-FKHR chimeric transcription factor generated by the t(2;13) translocation in alveolar rhabdomyosarcoma (ARMS) retains the PAX3 paired box (PB) and homeodomain (HD) DNA binding motifs, has a disrupted forkhead (FD) DNA binding domain, and acquires a COOH-terminal FKHR-derived activation domain.	bind
80234	7	3280	11	NULL	NULL	0	NULL	PAX3 paired box	PartOfProtein		is a type of 					DNA binding motif	PartOfProtein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_14_5019_s_31	10866659	(A) The PAX3-FKHR chimeric transcription factor generated by the t(2;13) translocation in alveolar rhabdomyosarcoma (ARMS) retains the PAX3 paired box (PB) and homeodomain (HD) DNA binding motifs, has a disrupted forkhead (FD) DNA binding domain, and acquires a COOH-terminal FKHR-derived activation domain.	bind
80235	8	3280	11	NULL	NULL	0	NULL	homeodomain	PartOfProtein		is a type of 					DNA binding motif	PartOfProtein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_14_5019_s_31	10866659	(A) The PAX3-FKHR chimeric transcription factor generated by the t(2;13) translocation in alveolar rhabdomyosarcoma (ARMS) retains the PAX3 paired box (PB) and homeodomain (HD) DNA binding motifs, has a disrupted forkhead (FD) DNA binding domain, and acquires a COOH-terminal FKHR-derived activation domain.	bind
80236	9	3280	11	NULL	NULL	0	NULL	PAX3-FKHR chimeric transcription factor	Protein		has 					forkhead DNA binding domain	PartOfProtein	disrupted			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_14_5019_s_31	10866659	(A) The PAX3-FKHR chimeric transcription factor generated by the t(2;13) translocation in alveolar rhabdomyosarcoma (ARMS) retains the PAX3 paired box (PB) and homeodomain (HD) DNA binding motifs, has a disrupted forkhead (FD) DNA binding domain, and acquires a COOH-terminal FKHR-derived activation domain.	bind
80237	10	3280	11	NULL	NULL	0	NULL	PAX3-FKHR chimeric transcription factor	Protein		acquires					FKHR-derived activation domain			COOH-terminal		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_14_5019_s_31	10866659	(A) The PAX3-FKHR chimeric transcription factor generated by the t(2;13) translocation in alveolar rhabdomyosarcoma (ARMS) retains the PAX3 paired box (PB) and homeodomain (HD) DNA binding motifs, has a disrupted forkhead (FD) DNA binding domain, and acquires a COOH-terminal FKHR-derived activation domain.	bind
8222	1	3281	5	11	NULL	0	NULL	peptide analogous to KCNK9	GP	wild-type	bind			N terminus		beta-COP	GP	rat;; brain			NULL		NULL	NULL	NULL	NULL	gw60_cell_111_4_577_s_170	12437930	(A) The peptide analogous to the wild-type N terminus of KCNK9 (and KCNK3) binds beta-COP from rat brain, while peptides with the NQ mutation do not (left).	bind
8223	2	3281	5	11	NULL	0	NULL	peptide analogous to KCNK3	GP	wild-type	bind			N terminus		beta-COP	GP	rat;; brain			NULL		NULL	NULL	NULL	NULL	gw60_cell_111_4_577_s_170	12437930	(A) The peptide analogous to the wild-type N terminus of KCNK9 (and KCNK3) binds beta-COP from rat brain, while peptides with the NQ mutation do not (left).	bind
8224	3	3281	5	11	NULL	0	NULL	peptide	GP	mutant	does not bind			NQ		beta-COP	GP	rat;; brain			NULL		NULL	NULL	NULL	NULL	gw60_cell_111_4_577_s_170	12437930	(A) The peptide analogous to the wild-type N terminus of KCNK9 (and KCNK3) binds beta-COP from rat brain, while peptides with the NQ mutation do not (left).	bind
10057	1	3281	7	11	NULL	0	NULL	peptide analogous to KCNK9	GP	wild-type	binds			N terminus		beta-COP	GP	rat;; brain			NULL		NULL	NULL	NULL	NULL	gw60_cell_111_4_577_s_170	12437930	(A) The peptide analogous to the wild-type N terminus of KCNK9 (and KCNK3) binds beta-COP from rat brain, while peptides with the NQ mutation do not (left).	bind
10058	2	3281	7	11	NULL	0	NULL	peptide analogous to KCNK3	GP	wild-type	bind			N terminus		beta-COP	GP	rat;; brain			NULL		NULL	NULL	NULL	NULL	gw60_cell_111_4_577_s_170	12437930	(A) The peptide analogous to the wild-type N terminus of KCNK9 (and KCNK3) binds beta-COP from rat brain, while peptides with the NQ mutation do not (left).	bind
10059	3	3281	7	11	NULL	0	NULL	peptides	GP	mutant	does not bind			NQ		beta-COP	GP	rat;; brain			NULL		NULL	NULL	NULL	NULL	gw60_cell_111_4_577_s_170	12437930	(A) The peptide analogous to the wild-type N terminus of KCNK9 (and KCNK3) binds beta-COP from rat brain, while peptides with the NQ mutation do not (left).	bind
80238	1	3281	11	NULL	NULL	0	NULL	 peptide analog 	PartOfProtein	wild-type KCNK9	binds to 			N terminus		beta-COP	Protein	rat brain			NULL		0	NULL	NULL	NULL	gw60_cell_111_4_577_s_170	12437930	(A) The peptide analogous to the wild-type N terminus of KCNK9 (and KCNK3) binds beta-COP from rat brain, while peptides with the NQ mutation do not (left).	bind
80239	2	3281	11	NULL	NULL	0	NULL	peptide analog	PartOfProtein	wild-type KCNK3	binds to 			N terminus		beta-COP	Protein	rat brain			NULL		0	NULL	NULL	NULL	gw60_cell_111_4_577_s_170	12437930	(A) The peptide analogous to the wild-type N terminus of KCNK9 (and KCNK3) binds beta-COP from rat brain, while peptides with the NQ mutation do not (left).	bind
80240	3	3281	11	NULL	NULL	0	NULL	peptides	PartOfProtein	NQ mutation	does not bind to					beta-COP	Protein	rat brain			NULL		0	NULL	NULL	NULL	gw60_cell_111_4_577_s_170	12437930	(A) The peptide analogous to the wild-type N terminus of KCNK9 (and KCNK3) binds beta-COP from rat brain, while peptides with the NQ mutation do not (left).	bind
80241	1	3283	11	NULL	NULL	0	NULL	GAL4 DNA binding site	PartOfProtein		is upstream of					SNRPN promoter	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_14_5107_s_224	10866667	(A) The reporter construct contains five copies of the GAL4 DNA binding site (5 x GAL) upstream of the  SNRPN promoter.	bind
8226	1	3288	5	11	NULL	0	NULL	p65	GP		bind		specifically			IkappaBalpha	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_3_1038_s_210	16428456	(A) The specificity of binding of p65 to IkappaBalpha and Bcl-X promoters.	bind
8227	2	3288	5	11	NULL	0	NULL	p65	GP		bind		specifically			Bcl-X	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_3_1038_s_210	16428456	(A) The specificity of binding of p65 to IkappaBalpha and Bcl-X promoters.	bind
10060	1	3288	7	11	NULL	0	NULL	p65 	GP		binds		specifically			IkappaBalpha	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_3_1038_s_210	16428456	(A) The specificity of binding of p65 to IkappaBalpha and Bcl-X promoters.	bind
10061	2	3288	7	11	NULL	0	NULL	p65	GP		binds		specifically			 Bcl-X 	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_3_1038_s_210	16428456	(A) The specificity of binding of p65 to IkappaBalpha and Bcl-X promoters.	bind
80242	1	3288	11	NULL	NULL	NULL	NULL	p65	Protein		binds to 					IkappaBalpha promoter	NucleicAcidSubstance				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_3_1038_s_210	16428456	(A) The specificity of binding of p65 to IkappaBalpha and Bcl-X promoters.	bind
80243	2	3288	11	NULL	NULL	0	NULL	p65	Protein		binds to 					Bcl-X promoter	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_3_1038_s_210	16428456	(A) The specificity of binding of p65 to IkappaBalpha and Bcl-X promoters.	bind
80244	1	3289	11	NULL	NULL	NULL	NULL	Pol II	Protein		binds to 					GAL10 promoter	NucleicAcidSubstance	induced			NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_5_1301_s_133	12769853	(A) The strain was deleted for  spt20, and the binding of Pol II and of the Mediator were measured at the  GAL10 (Gal1p13i; see Experimental Procedures) promoter following induction.	bind
8378	1	3290	5	11	NULL	0	NULL	betaPIX	GP		bind			N-terminal SH3 domain		PAK	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6354_s_160	10938112	(A) The structural domains of betaPIX include its N-terminal SH3 domain, which binds PAK, a catalytic Dbl homology (DH) region promoting nucleotide exchange on Rac1, and a C-terminal region (bar) which was used to bind GIT1 (B) by overlay.	bind
8379	2	3290	5	11	NULL	0	NULL	betaPIX	GP	catalytic	promote			DH		Rac1	GP	nucleotide exchange on			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6354_s_160	10938112	(A) The structural domains of betaPIX include its N-terminal SH3 domain, which binds PAK, a catalytic Dbl homology (DH) region promoting nucleotide exchange on Rac1, and a C-terminal region (bar) which was used to bind GIT1 (B) by overlay.	bind
8380	3	3290	5	11	NULL	0	NULL	DH	GP		is					Dbl homology region	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6354_s_160	10938112	(A) The structural domains of betaPIX include its N-terminal SH3 domain, which binds PAK, a catalytic Dbl homology (DH) region promoting nucleotide exchange on Rac1, and a C-terminal region (bar) which was used to bind GIT1 (B) by overlay.	bind
8381	4	3290	5	11	NULL	0	NULL	betaPIX	GP		bind			C-terminal region		GIT1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6354_s_160	10938112	(A) The structural domains of betaPIX include its N-terminal SH3 domain, which binds PAK, a catalytic Dbl homology (DH) region promoting nucleotide exchange on Rac1, and a C-terminal region (bar) which was used to bind GIT1 (B) by overlay.	bind
10062	1	3290	7	11	NULL	0	NULL	betaPIX	GP		binds			N-terminal SH3 domain		PAK	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6354_s_160	10938112	(A) The structural domains of betaPIX include its N-terminal SH3 domain, which binds PAK, a catalytic Dbl homology (DH) region promoting nucleotide exchange on Rac1, and a C-terminal region (bar) which was used to bind GIT1 (B) by overlay.	bind
10063	2	3290	7	11	NULL	0	NULL	betaPIX	GP		binds			C-terminal region		GIT1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6354_s_160	10938112	(A) The structural domains of betaPIX include its N-terminal SH3 domain, which binds PAK, a catalytic Dbl homology (DH) region promoting nucleotide exchange on Rac1, and a C-terminal region (bar) which was used to bind GIT1 (B) by overlay.	bind
10064	3	3290	7	11	NULL	0	NULL	betaPIX	GP	catalytic	promote			 Dbl homology region		Rac1	GP	nucleotide exchange on			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6354_s_160	10938112	(A) The structural domains of betaPIX include its N-terminal SH3 domain, which binds PAK, a catalytic Dbl homology (DH) region promoting nucleotide exchange on Rac1, and a C-terminal region (bar) which was used to bind GIT1 (B) by overlay.	bind
12394	4	3290	7	11	NULL	0	NULL	Dbl homology region	GP		is					DH	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6354_s_160	10938112	(A) The structural domains of betaPIX include its N-terminal SH3 domain, which binds PAK, a catalytic Dbl homology (DH) region promoting nucleotide exchange on Rac1, and a C-terminal region (bar) which was used to bind GIT1 (B) by overlay.	bind
80245	1	3290	11	NULL	NULL	NULL	NULL	betaPIX	Protein		binds to 			N-terminal SH3 domain		PAK	Protein				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6354_s_160	10938112	(A) The structural domains of betaPIX include its N-terminal SH3 domain, which binds PAK, a catalytic Dbl homology (DH) region promoting nucleotide exchange on Rac1, and a C-terminal region (bar) which was used to bind GIT1 (B) by overlay.	bind
80246	2	3290	11	NULL	NULL	0	NULL	PAK	Protein		exchange		nucleotide	catalytic Dbl homology region		Rac1	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_17_6354_s_160	10938112	(A) The structural domains of betaPIX include its N-terminal SH3 domain, which binds PAK, a catalytic Dbl homology (DH) region promoting nucleotide exchange on Rac1, and a C-terminal region (bar) which was used to bind GIT1 (B) by overlay.	bind
80247	3	3290	11	NULL	NULL	0	NULL	PAK	Protein	 C-terminal 	binds to 					GIT1	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_17_6354_s_160	10938112	(A) The structural domains of betaPIX include its N-terminal SH3 domain, which binds PAK, a catalytic Dbl homology (DH) region promoting nucleotide exchange on Rac1, and a C-terminal region (bar) which was used to bind GIT1 (B) by overlay.	bind
8385	1	3291	5	11	NULL	0	NULL	DIAP1-BIR2	GP		bind					Skl peptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_2_125_s_130	11818063	(A) The structure of a DIAP1-BIR2 (cyan) bound to a Skl peptide (green) is superimposed with that complexed with a Hid (pink) or Grim (orange) peptide.	bind
10065	1	3291	7	11	NULL	0	NULL	DIAP1-BIR2	GP		bind					Skl peptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_2_125_s_130	11818063	(A) The structure of a DIAP1-BIR2 (cyan) bound to a Skl peptide (green) is superimposed with that complexed with a Hid (pink) or Grim (orange) peptide.	bind
80248	1	3291	11	NULL	NULL	0	NULL	DIAP1-BIR2	Protein		binds to 					Skl peptide	PartOfProtein				NULL		0	NULL	NULL	NULL	gw60_currbiol_12_2_125_s_130	11818063	(A) The structure of a DIAP1-BIR2 (cyan) bound to a Skl peptide (green) is superimposed with that complexed with a Hid (pink) or Grim (orange) peptide.	bind
80249	2	3291	11	NULL	NULL	0	NULL	Skl peptide	PartOfProtein		complexed with					Hid peptide	PartOfProtein				NULL		0	NULL	NULL	NULL	gw60_currbiol_12_2_125_s_130	11818063	(A) The structure of a DIAP1-BIR2 (cyan) bound to a Skl peptide (green) is superimposed with that complexed with a Hid (pink) or Grim (orange) peptide.	bind
80250	3	3291	11	NULL	NULL	0	NULL	Skl peptide	PartOfProtein		complexed with					Grim peptide	PartOfProtein				NULL		0	NULL	NULL	NULL	gw60_currbiol_12_2_125_s_130	11818063	(A) The structure of a DIAP1-BIR2 (cyan) bound to a Skl peptide (green) is superimposed with that complexed with a Hid (pink) or Grim (orange) peptide.	bind
8386	1	3292	5	11	NULL	0	NULL	PI3K	GP		bind					ATP	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_6_931_s_274	11136978	(A) The structure of PI3K  bound to ATP is traced through the C  s  as a black dotted line.	bind
10068	1	3292	7	11	NULL	0	NULL	PI3K 	GP		binds					ATP	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_6_931_s_274	11136978	(A) The structure of PI3K  bound to ATP is traced through the C  s  as a black dotted line.	bind
80251	1	3292	11	NULL	NULL	0	NULL	PI3K	Protein		binds to 					ATP	Chemical				NULL		0	NULL	NULL	NULL	gw60_cell_103_6_931_s_274	11136978	(A) The structure of PI3K  bound to ATP is traced through the C  s  as a black dotted line.	bind
8387	1	3293	5	11	NULL	0	NULL	tRNAVal	NucleicAcid		bind			CCA region					editing domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_103_5_793_s_147	11114335	(A) The tRNAVal CCA region is bound to  the editing domain.	bind
10069	1	3293	7	11	NULL	0	NULL	tRNAVal	NucleicAcid		binds			CCA region					editing domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_103_5_793_s_147	11114335	(A) The tRNAVal CCA region is bound to  the editing domain.	bind
80252	1	3293	11	NULL	NULL	0	NULL	tRNAVal	NucleicAcidSubstance	CCA region	binds to 								editing domain		NULL		0	NULL	NULL	NULL	gw60_cell_103_5_793_s_147	11114335	(A) The tRNAVal CCA region is bound to  the editing domain.	bind
8388	1	3294	5	11	NULL	0	NULL	FGFR2	GP	two-loop form of	bind		marginal affinity			FGF-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_6754_s_367	10490614	(A) The two-loop form of FGFR2, deltaAD, binds to FGF-1 with marginal affinity and transmits weak downstream signals.	bind
8389	2	3294	5	11	NULL	0	NULL				bind		marginal affinity	deltaAD		FGF-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_6754_s_367	10490614	(A) The two-loop form of FGFR2, deltaAD, binds to FGF-1 with marginal affinity and transmits weak downstream signals.	bind
10070	1	3294	7	11	NULL	0	NULL	FGFR2	GP	two-loop form of	binds		with marginal affinity	deltaAD		FGF-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_6754_s_367	10490614	(A) The two-loop form of FGFR2, deltaAD, binds to FGF-1 with marginal affinity and transmits weak downstream signals.	bind
12401	2	3294	7	11	NULL	0	NULL	statement 1	GP		transmits					weak downstream signals					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_6754_s_367	10490614	(A) The two-loop form of FGFR2, deltaAD, binds to FGF-1 with marginal affinity and transmits weak downstream signals.	bind
80253	1	3294	11	NULL	NULL	0	NULL	FGFR2	Protein	two-loop form	binds to 		marginal affinity			FGF-1	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_10_6754_s_367	10490614	(A) The two-loop form of FGFR2, deltaAD, binds to FGF-1 with marginal affinity and transmits weak downstream signals.	bind
80254	2	3294	11	NULL	NULL	0	NULL	deltaAD	PartOfProtein		binds to 		marginal affinity			FGF-1	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_10_6754_s_367	10490614	(A) The two-loop form of FGFR2, deltaAD, binds to FGF-1 with marginal affinity and transmits weak downstream signals.	bind
80255	3	3294	11	NULL	NULL	0	NULL	statement 1	Process		transmits					downstream signals	MolecularProcess	weak			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_10_6754_s_367	10490614	(A) The two-loop form of FGFR2, deltaAD, binds to FGF-1 with marginal affinity and transmits weak downstream signals.	bind
80256	4	3294	11	NULL	NULL	0	NULL	statement 2	Process		transmits					downstream signals	MolecularProcess	weak			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_10_6754_s_367	10490614	(A) The two-loop form of FGFR2, deltaAD, binds to FGF-1 with marginal affinity and transmits weak downstream signals.	bind
8392	1	3295	5	11	NULL	0	NULL	Vg1	GP		bind				LS	similar oocyte factors	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_10_4669_s_235	15292452	(A) The Vg1 LS and Xcat2 3'UTR bind  to similar oocyte factors.	bind
8393	2	3295	5	11	NULL	0	NULL	Xcat2	GP		bind				3'UTR	similar oocyte factors	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_10_4669_s_235	15292452	(A) The Vg1 LS and Xcat2 3'UTR bind  to similar oocyte factors.	bind
10071	1	3295	7	11	NULL	0	NULL	Vg1 	GP		bind				LS	oocyte factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_10_4669_s_235	15292452	(A) The Vg1 LS and Xcat2 3'UTR bind  to similar oocyte factors.	bind
10072	2	3295	7	11	NULL	0	NULL	Xcat2 	GP		bind				3'UTR	oocyte factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_10_4669_s_235	15292452	(A) The Vg1 LS and Xcat2 3'UTR bind  to similar oocyte factors.	bind
80257	1	3295	11	NULL	NULL	0	NULL	Vg1 LS	NucleicAcidSubstance		binds to 				3'UTR	oocyte factor	Protein				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_10_4669_s_235	15292452	(A) The Vg1 LS and Xcat2 3'UTR bind  to similar oocyte factors.	bind
80258	2	3295	11	NULL	NULL	0	NULL	Xcat2	NucleicAcidSubstance		binds to 				3'UTR	oocyte factor	Protein				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_10_4669_s_235	15292452	(A) The Vg1 LS and Xcat2 3'UTR bind  to similar oocyte factors.	bind
8394	1	3296	5	11	NULL	0	NULL	MIM	GP		bind		specifically	WH2 domain		G-actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_3_453_s_113	15684034	(A) The WH2 domain of MIM specifically binds G-actin.	bind
10073	1	3296	7	11	NULL	0	NULL	MIM	GP		binds		specifically	WH2 domain		G-actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_3_453_s_113	15684034	(A) The WH2 domain of MIM specifically binds G-actin.	bind
80259	1	3296	11	NULL	NULL	0	NULL	MIM	Protein		binds to 		specifically	WH2 domain		G-actin	Protein				NULL		0	NULL	NULL	NULL	gw70_cellbiol_168_3_453_s_113	15684034	(A) The WH2 domain of MIM specifically binds G-actin.	bind
8395	1	3297	5	11	NULL	0	NULL	BP-1	GP		bind					E1B 19K	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4390_s_131	10330179	(A) The yeast two-hybrid assay was used to demonstrate binding between BP-1 and E1B 19K.	bind
10074	1	3297	7	11	NULL	0	NULL	BP-1	GP		binds					E1B 19K	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4390_s_131	10330179	(A) The yeast two-hybrid assay was used to demonstrate binding between BP-1 and E1B 19K.	bind
80267	1	3297	11	NULL	NULL	0	NULL	BP-1	Protein		binds to 					E1B	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_6_4390_s_131	10330179	(A) The yeast two-hybrid assay was used to demonstrate binding between BP-1 and E1B 19K.	bind
8396	1	3298	5	11	NULL	0	NULL	Yop-specific chaperone	GP		bind					cognate Yop protein	GP		translocation domain		NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_62_2_379_s_730	9618447	(A) The Yop-specific chaperone binds to the translocation domain of its cognate Yop protein.	bind
10075	1	3298	7	11	NULL	0	NULL	Yop-specific chaperone	GP		binds					Yop protein	GP		translocation domain		NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_62_2_379_s_730	9618447	(A) The Yop-specific chaperone binds to the translocation domain of its cognate Yop protein.	bind
80268	1	3298	11	NULL	NULL	0	NULL	Yop-specific chaperone	Protein		binds to 					cognate Yop protein	Protein		translocation domain		NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_62_2_379_s_730	9618447	(A) The Yop-specific chaperone binds to the translocation domain of its cognate Yop protein.	bind
8397	1	3299	5	11	NULL	0	NULL	THP-1 cell	Cell		bind					von Willebrand factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_153_5_905_s_236	11381078	(A) THP-1 cell binding to von Willebrand factor was examined in the presence of antibodies against the beta2 (7E4), alphaVbeta3 (LM609), or alphaIIbbeta3 (P2) integrins.	bind
10076	1	3299	7	11	NULL	0	NULL	THP-1 cell 	Cell		binds					von Willebrand factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_153_5_905_s_236	11381078	(A) THP-1 cell binding to von Willebrand factor was examined in the presence of antibodies against the beta2 (7E4), alphaVbeta3 (LM609), or alphaIIbbeta3 (P2) integrins.	bind
80269	1	3299	11	NULL	NULL	0	NULL	THP-1 cell	cell		binds to 					von Willebrand factor	Protein				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_5_905_s_236	11381078	(A) THP-1 cell binding to von Willebrand factor was examined in the presence of antibodies against the beta2 (7E4), alphaVbeta3 (LM609), or alphaIIbbeta3 (P2) integrins.	bind
8398	1	3302	5	11	NULL	0	NULL	poly-L-proline	AminoAcid		bind							mutant	Y5D		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_274	11294914	(A) Time course of polymerization of actin alone ( ) and with wild-type profilin ( ), poly-L-proline binding mutant Y5D ( ), and actin binding mutants Y79R ( ), K81F ( ), and P107W ( ).	bind
8399	2	3302	5	11	NULL	0	NULL	actin	GP		bind							mutant	Y79R		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_274	11294914	(A) Time course of polymerization of actin alone ( ) and with wild-type profilin ( ), poly-L-proline binding mutant Y5D ( ), and actin binding mutants Y79R ( ), K81F ( ), and P107W ( ).	bind
8400	3	3302	5	11	NULL	0	NULL	actin	GP		bind							mutant	K81F		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_274	11294914	(A) Time course of polymerization of actin alone ( ) and with wild-type profilin ( ), poly-L-proline binding mutant Y5D ( ), and actin binding mutants Y79R ( ), K81F ( ), and P107W ( ).	bind
8401	4	3302	5	11	NULL	0	NULL	actin	GP		bind							mutant	P107W		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_274	11294914	(A) Time course of polymerization of actin alone ( ) and with wild-type profilin ( ), poly-L-proline binding mutant Y5D ( ), and actin binding mutants Y79R ( ), K81F ( ), and P107W ( ).	bind
11725	1	3302	7	11	NULL	0	NULL	 poly-L-proline	AminoAcid		bind							mutant	Y5D		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_274	11294914	(A) Time course of polymerization of actin alone ( ) and with wild-type profilin ( ), poly-L-proline binding mutant Y5D ( ), and actin binding mutants Y79R ( ), K81F ( ), and P107W ( ).	bind
11726	2	3302	7	11	NULL	0	NULL	actin	GP		bind							mutant	Y79R		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_274	11294914	(A) Time course of polymerization of actin alone ( ) and with wild-type profilin ( ), poly-L-proline binding mutant Y5D ( ), and actin binding mutants Y79R ( ), K81F ( ), and P107W ( ).	bind
11727	3	3302	7	11	NULL	0	NULL	actin	GP		bind							mutant	K81F		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_274	11294914	(A) Time course of polymerization of actin alone ( ) and with wild-type profilin ( ), poly-L-proline binding mutant Y5D ( ), and actin binding mutants Y79R ( ), K81F ( ), and P107W ( ).	bind
11728	4	3302	7	11	NULL	0	NULL	actin	GP		bind							mutant	P107W		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_274	11294914	(A) Time course of polymerization of actin alone ( ) and with wild-type profilin ( ), poly-L-proline binding mutant Y5D ( ), and actin binding mutants Y79R ( ), K81F ( ), and P107W ( ).	bind
80270	1	3302	11	NULL	NULL	0	NULL	poly-L-proline	AminoAcid		binds to 					Y5D	PartOfProtein	 mutant			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_274	11294914	(A) Time course of polymerization of actin alone ( ) and with wild-type profilin ( ), poly-L-proline binding mutant Y5D ( ), and actin binding mutants Y79R ( ), K81F ( ), and P107W ( ).	bind
80271	2	3302	11	NULL	NULL	0	NULL	actin	Protein		binds to 					Y79R	PartOfProtein	mutant			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_274	11294914	(A) Time course of polymerization of actin alone ( ) and with wild-type profilin ( ), poly-L-proline binding mutant Y5D ( ), and actin binding mutants Y79R ( ), K81F ( ), and P107W ( ).	bind
80272	3	3302	11	NULL	NULL	0	NULL	actin	Protein		binds to 					K81F	PartOfProtein	mutant			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_274	11294914	(A) Time course of polymerization of actin alone ( ) and with wild-type profilin ( ), poly-L-proline binding mutant Y5D ( ), and actin binding mutants Y79R ( ), K81F ( ), and P107W ( ).	bind
80273	4	3302	11	NULL	NULL	0	NULL	actin	Protein		binds to 					P107W	PartOfProtein	mutant			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_274	11294914	(A) Time course of polymerization of actin alone ( ) and with wild-type profilin ( ), poly-L-proline binding mutant Y5D ( ), and actin binding mutants Y79R ( ), K81F ( ), and P107W ( ).	bind
8402	1	3303	5	11	NULL	0	NULL	GTP S	Chemical		bind					ARF	GP	bovine			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_6_387_s_43	9197239	(a) Time course of the binding of GTP  S to bovine ARF.	bind
10295	1	3303	7	11	NULL	0	NULL	GTP S 	Chemical		bind					ARF	GP	bovine			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_6_387_s_43	9197239	(a) Time course of the binding of GTP  S to bovine ARF.	bind
80274	1	3303	11	NULL	NULL	0	NULL	ARF	Protein	bovine	binds to 					GTP S	Chemical				NULL		0	NULL	NULL	NULL	gw60_currbiol_7_6_387_s_43	9197239	(a) Time course of the binding of GTP  S to bovine ARF.	bind
10299	1	3304	7	11	NULL	0	NULL	Trx-PreS	GP		bind					HBcAg-coated wells					NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_319_3_959_s_121	15184075	(A) Time-course of Trx-PreS binding to HBcAg-coated wells.	bind
80275	1	3304	11	NULL	NULL	0	NULL	Trx-PreS	Chemical		binds to 					wells	Thing	HBcAg-coated			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_319_3_959_s_121	15184075	(A) Time-course of Trx-PreS binding to HBcAg-coated wells.	bind
8403	1	3305	5	11	NULL	0	NULL	BMP2	GP		activate					p38 kinase	GP				NULL	C3H10T1/2	NULL	NULL	NULL	NULL	gw60_molbiolcell_14_2_545_s_174	12589053	(A) Time-dependent activation of p38 kinase by BMP2 in C3H10T1/2.	bind
10302	1	3305	7	11	NULL	0	NULL	BMP2	GP		activate					p38 kinase	GP				NULL	C3H10T1/2	NULL	NULL	NULL	NULL	gw60_molbiolcell_14_2_545_s_174	12589053	(A) Time-dependent activation of p38 kinase by BMP2 in C3H10T1/2.	bind
80276	1	3305	11	NULL	NULL	0	NULL	 BMP2	Protein		binds to 					p38 kinase	Protein				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_2_545_s_174	12589053	(A) Time-dependent activation of p38 kinase by BMP2 in C3H10T1/2.	bind
8405	1	3306	5	11	NULL	0	NULL	GDP	Chemical		bind					RF3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_4_789_s_175	12419223	(A) Time-dependent exchange of RF3-bound [3]GDP to cold GDP is catalyzed by mutant and wild-type factors bound to the ribosome.	bind
8406	2	3306	5	11	NULL	0	NULL	statement 1	Chemical		is exchanged with					GDP	Chemical	cold 			NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_4_789_s_175	12419223	(A) Time-dependent exchange of RF3-bound [3]GDP to cold GDP is catalyzed by mutant and wild-type factors bound to the ribosome.	bind
8407	3	3306	5	11	NULL	0	NULL	factors	GP	wild-type	bind					ribosomes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_4_789_s_175	12419223	(A) Time-dependent exchange of RF3-bound [3]GDP to cold GDP is catalyzed by mutant and wild-type factors bound to the ribosome.	bind
8408	4	3306	5	11	NULL	0	NULL	factors	GP	mutant	bind					ribosomes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_4_789_s_175	12419223	(A) Time-dependent exchange of RF3-bound [3]GDP to cold GDP is catalyzed by mutant and wild-type factors bound to the ribosome.	bind
8409	5	3306	5	11	NULL	0	NULL	statement 3	Process		catalyze					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_4_789_s_175	12419223	(A) Time-dependent exchange of RF3-bound [3]GDP to cold GDP is catalyzed by mutant and wild-type factors bound to the ribosome.	bind
8410	6	3306	5	11	NULL	0	NULL	statement 4	Process		catalyze					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_4_789_s_175	12419223	(A) Time-dependent exchange of RF3-bound [3]GDP to cold GDP is catalyzed by mutant and wild-type factors bound to the ribosome.	bind
10303	1	3306	7	11	NULL	0	NULL	RF3-bound [3]GDP	GP		exchange					GDP	Chemical	cold			NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_4_789_s_175	12419223	(A) Time-dependent exchange of RF3-bound [3]GDP to cold GDP is catalyzed by mutant and wild-type factors bound to the ribosome.	bind
10304	2	3306	7	11	NULL	0	NULL	statement 1	Process		is catalysed by					factors bound to ribosome	CellComponent	mutant			NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_4_789_s_175	12419223	(A) Time-dependent exchange of RF3-bound [3]GDP to cold GDP is catalyzed by mutant and wild-type factors bound to the ribosome.	bind
10305	3	3306	7	11	NULL	0	NULL	statement 1	Process		is catalysed by					factors bound to ribosome	CellComponent	wild-type			NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_4_789_s_175	12419223	(A) Time-dependent exchange of RF3-bound [3]GDP to cold GDP is catalyzed by mutant and wild-type factors bound to the ribosome.	bind
80281	1	3306	11	NULL	NULL	0	NULL	RF3	Protein		binds to 					GDP	Chemical				NULL		0	NULL	NULL	NULL	gw60_molcell_10_4_789_s_175	12419223	(A) Time-dependent exchange of RF3-bound [3]GDP to cold GDP is catalyzed by mutant and wild-type factors bound to the ribosome.	bind
80282	2	3306	11	NULL	NULL	0	NULL	wild-type factors	Thing		binds to 					ribosome	CellComponent				NULL		0	NULL	NULL	NULL	gw60_molcell_10_4_789_s_175	12419223	(A) Time-dependent exchange of RF3-bound [3]GDP to cold GDP is catalyzed by mutant and wild-type factors bound to the ribosome.	bind
80283	3	3306	11	NULL	NULL	0	NULL	mutant factors	Thing		binds to 					ribosome	CellComponent				NULL		0	NULL	NULL	NULL	gw60_molcell_10_4_789_s_175	12419223	(A) Time-dependent exchange of RF3-bound [3]GDP to cold GDP is catalyzed by mutant and wild-type factors bound to the ribosome.	bind
80284	4	3306	11	NULL	NULL	0	NULL	statement 1	Process		exchange to		Time-dependent			GDP	Chemical	cold			NULL		0	NULL	NULL	NULL	gw60_molcell_10_4_789_s_175	12419223	(A) Time-dependent exchange of RF3-bound [3]GDP to cold GDP is catalyzed by mutant and wild-type factors bound to the ribosome.	bind
80285	5	3306	11	NULL	NULL	0	NULL	statement 2	Thing		catalyzes					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_10_4_789_s_175	12419223	(A) Time-dependent exchange of RF3-bound [3]GDP to cold GDP is catalyzed by mutant and wild-type factors bound to the ribosome.	bind
80286	6	3306	11	NULL	NULL	0	NULL	statement 3	Thing		catalyzes					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_10_4_789_s_175	12419223	(A) Time-dependent exchange of RF3-bound [3]GDP to cold GDP is catalyzed by mutant and wild-type factors bound to the ribosome.	bind
8411	1	3307	5	11	NULL	0	NULL	melittin	GP		bind					POPC membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1665_1_29_s_148	15471568	(a) Time-resolved fluorescence intensity decay of melittin bound to POPC membranes.	bind
10308	1	3307	7	11	NULL	0	NULL	melittin	GP		bind					POPC membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1665_1_29_s_148	15471568	(a) Time-resolved fluorescence intensity decay of melittin bound to POPC membranes.	bind
80287	1	3307	11	NULL	NULL	0	NULL	melittin	Protein		binds to 					membranes	CellComponent	POPC 			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1665_1_29_s_148	15471568	(a) Time-resolved fluorescence intensity decay of melittin bound to POPC membranes.	bind
8412	1	3308	5	11	NULL	0	NULL	GDP	Chemical		bind					NDP kinase B	GP	wild type;; human			NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_63_3_538_s_147	12606760	(A) to d4T triphosphate (green) bound  to the same protein in the 1.85  Ang  resolution structure determined by (Meyer et al.,  2000 ) in (B), to GDP bound to wild type human NDP kinase B (Morera et al., 1995 ).	bind
10314	1	3308	7	11	NULL	0	NULL	GDP	Chemical		bind					NDP kinase B 	GP	wild type;; human			NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_63_3_538_s_147	12606760	(A) to d4T triphosphate (green) bound  to the same protein in the 1.85  Ang  resolution structure determined by (Meyer et al.,  2000 ) in (B), to GDP bound to wild type human NDP kinase B (Morera et al., 1995 ).	bind
80288	1	3308	11	NULL	NULL	0	NULL	GDP	Chemical		binds to 					NDP kinase B 	Protein	wild type;;human			NULL		0	NULL	NULL	NULL	gw70_molpharmacol_63_3_538_s_147	12606760	(A) to d4T triphosphate (green) bound  to the same protein in the 1.85  Ang  resolution structure determined by (Meyer et al.,  2000 ) in (B), to GDP bound to wild type human NDP kinase B (Morera et al., 1995 ).	bind
8413	1	3312	5	11	NULL	0	NULL	pp F			bind					Sec complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_94_6_795_s_36	9753326	(A) To probe  the environment of pp F bound to the Sec complex by cross-linking, the indicated  lysine residues (K) were replaced by photoreactive lysine derivatives.	bind
10315	1	3312	7	11	NULL	0	NULL	pp F			bind					Sec complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_94_6_795_s_36	9753326	(A) To probe  the environment of pp F bound to the Sec complex by cross-linking, the indicated  lysine residues (K) were replaced by photoreactive lysine derivatives.	bind
80289	1	3312	11	NULL	NULL	0	NULL	pp&#945;F 	Protein		binds to 		 cross-linking			Sec complex	Protein				NULL		0	NULL	NULL	NULL	gw60_cell_94_6_795_s_36	9753326	(A) To probe  the environment of pp F bound to the Sec complex by cross-linking, the indicated  lysine residues (K) were replaced by photoreactive lysine derivatives.	bind
80290	2	3312	11	NULL	NULL	0	NULL	 lysine residue	AminoAcid		is					K	AminoAcid				NULL		0	NULL	NULL	NULL	gw60_cell_94_6_795_s_36	9753326	(A) To probe  the environment of pp F bound to the Sec complex by cross-linking, the indicated  lysine residues (K) were replaced by photoreactive lysine derivatives.	bind
80291	3	3312	11	NULL	NULL	0	NULL	 lysine residue	AminoAcid		replaced by					lysine derivative	AminoAcid	photoreactive			NULL		0	NULL	NULL	NULL	gw60_cell_94_6_795_s_36	9753326	(A) To probe  the environment of pp F bound to the Sec complex by cross-linking, the indicated  lysine residues (K) were replaced by photoreactive lysine derivatives.	bind
8414	1	3313	5	11	NULL	0	NULL	Tollip	GP		bind					IRAK	GP				NULL	HEK293T cells	NULL	NULL	NULL	NULL	gw70_febslett_575_1_136_s_123	15388348	(A) Tollip binds to IRAK in an immunoprecipitation  assay in HEK293T cells.	bind
10318	1	3313	7	11	NULL	0	NULL	Tollip	GP		binds					 IRAK	GP				NULL	HEK293T cells	NULL	NULL	NULL	NULL	gw70_febslett_575_1_136_s_123	15388348	(A) Tollip binds to IRAK in an immunoprecipitation  assay in HEK293T cells.	bind
80292	1	3313	11	NULL	NULL	0	NULL	Tollip	Protein		binds to 					IRAK	Protein				NULL	HEK293T cells	0	NULL	NULL	NULL	gw70_febslett_575_1_136_s_123	15388348	(A) Tollip binds to IRAK in an immunoprecipitation  assay in HEK293T cells.	bind
80293	2	3313	11	NULL	NULL	0	NULL	statement 1	Process		happens in					immunoprecipitation assay	ResearchActivity				NULL		0	NULL	NULL	NULL	gw70_febslett_575_1_136_s_123	15388348	(A) Tollip binds to IRAK in an immunoprecipitation  assay in HEK293T cells.	bind
8415	1	3314	5	11	NULL	0	NULL	HEK cells	Cell		transfected with					AChR cDNAs	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_17_1_157_s_134	8755487	(A) Total  -bgt binding to intact HEK cells transfected with the indicated AChR cDNAs.	bind
8416	2	3314	5	11	NULL	0	NULL	Total -bgt	Chemical		bind					statement 1	Cell				NULL		NULL	NULL	NULL	NULL	gw60_neuron_17_1_157_s_134	8755487	(A) Total  -bgt binding to intact HEK cells transfected with the indicated AChR cDNAs.	bind
10321	2	3314	7	11	NULL	0	NULL	Total -bgt	Chemical		bind					statement 1	Cell				NULL		NULL	NULL	NULL	NULL	gw60_neuron_17_1_157_s_134	8755487	(A) Total  -bgt binding to intact HEK cells transfected with the indicated AChR cDNAs.	bind
10323	1	3314	7	11	NULL	0	NULL	HEK cells	Cell		is transfected with					AChR cDNA	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_17_1_157_s_134	8755487	(A) Total  -bgt binding to intact HEK cells transfected with the indicated AChR cDNAs.	bind
80294	1	3314	11	NULL	NULL	0	NULL	HEK cells	cell	intact	transfected with					AChR cDNAs	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_neuron_17_1_157_s_134	8755487	(A) Total  -bgt binding to intact HEK cells transfected with the indicated AChR cDNAs.	bind
80295	2	3314	11	NULL	NULL	0	NULL	bgt	Protein		binds to 					statement 1	Cell				NULL		0	NULL	NULL	NULL	gw60_neuron_17_1_157_s_134	8755487	(A) Total  -bgt binding to intact HEK cells transfected with the indicated AChR cDNAs.	bind
8417	1	3315	5	11	NULL	0	NULL	rhotekin	GP		bind		specifically	Rho-binding domain		Rho	GP	activated			NULL	total cell extracts from mouse primary keratinocytes	NULL	NULL	NULL	NULL	gw60_cellbiol_156_1_137_s_33	11777936	(A) Total cell extracts from mouse primary keratinocytes under low calcium conditions and at various times of calcium exposure were incubated with beads coupled to the Rho-binding domain of rhotekin, which binds specifically to activated Rho.	bind
10344	1	3315	7	11	NULL	0	NULL	 rhotekin	GP		bind		specifically	Rho-binding domain 		Rho	GP	activated			NULL	cell extracts from mouse primary keratinocytes 	NULL	NULL	NULL	NULL	gw60_cellbiol_156_1_137_s_33	11777936	(A) Total cell extracts from mouse primary keratinocytes under low calcium conditions and at various times of calcium exposure were incubated with beads coupled to the Rho-binding domain of rhotekin, which binds specifically to activated Rho.	bind
80296	1	3315	11	NULL	NULL	0	NULL	rhotekin	Protein		has								Rho-binding domain 		NULL		0	NULL	NULL	NULL	gw60_cellbiol_156_1_137_s_33	11777936	(A) Total cell extracts from mouse primary keratinocytes under low calcium conditions and at various times of calcium exposure were incubated with beads coupled to the Rho-binding domain of rhotekin, which binds specifically to activated Rho.	bind
80297	2	3315	11	NULL	NULL	0	NULL	rhotekin	Protein		binds to 		specifically	Rho-binding domain 		Rho	Protein	activated			NULL		0	NULL	NULL	NULL	gw60_cellbiol_156_1_137_s_33	11777936	(A) Total cell extracts from mouse primary keratinocytes under low calcium conditions and at various times of calcium exposure were incubated with beads coupled to the Rho-binding domain of rhotekin, which binds specifically to activated Rho.	bind
8418	1	3316	5	11	NULL	0	NULL	Sfl1	GP		bind					FLO11	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_3981_s_355	12024012	(A) Tpk2 controls binding of Sfl1 and Flo8 to the  FLO11 promoter.	bind
8419	2	3316	5	11	NULL	0	NULL	Flo8	GP		bind					FLO11	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_3981_s_355	12024012	(A) Tpk2 controls binding of Sfl1 and Flo8 to the  FLO11 promoter.	bind
8420	3	3316	5	11	NULL	0	NULL	Tpk2	GP		control					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_3981_s_355	12024012	(A) Tpk2 controls binding of Sfl1 and Flo8 to the  FLO11 promoter.	bind
8421	4	3316	5	11	NULL	0	NULL	Tpk2	GP		control					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_3981_s_355	12024012	(A) Tpk2 controls binding of Sfl1 and Flo8 to the  FLO11 promoter.	bind
10345	1	3316	7	11	NULL	0	NULL	Sfl1	GP		bind					FLO11	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_3981_s_355	12024012	(A) Tpk2 controls binding of Sfl1 and Flo8 to the  FLO11 promoter.	bind
10346	2	3316	7	11	NULL	0	NULL	Flo8	GP		bind					FLO11	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_3981_s_355	12024012	(A) Tpk2 controls binding of Sfl1 and Flo8 to the  FLO11 promoter.	bind
10347	3	3316	7	11	NULL	0	NULL	Tpk2	GP		controls					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_3981_s_355	12024012	(A) Tpk2 controls binding of Sfl1 and Flo8 to the  FLO11 promoter.	bind
10348	4	3316	7	11	NULL	0	NULL	Tpk2	GP		controls					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_3981_s_355	12024012	(A) Tpk2 controls binding of Sfl1 and Flo8 to the  FLO11 promoter.	bind
80298	1	3316	11	NULL	NULL	0	NULL	Sfl1	Protein		binds to 					FLO11 promoter	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_12_3981_s_355	12024012	(A) Tpk2 controls binding of Sfl1 and Flo8 to the  FLO11 promoter.	bind
80299	2	3316	11	NULL	NULL	0	NULL	Flo8	Protein		binds to 					FLO11 promoter	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_12_3981_s_355	12024012	(A) Tpk2 controls binding of Sfl1 and Flo8 to the  FLO11 promoter.	bind
80300	3	3316	11	NULL	NULL	0	NULL	Tpk2	Protein		controls					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_12_3981_s_355	12024012	(A) Tpk2 controls binding of Sfl1 and Flo8 to the  FLO11 promoter.	bind
80301	4	3316	11	NULL	NULL	0	NULL	Tpk2	Protein		controls					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_12_3981_s_355	12024012	(A) Tpk2 controls binding of Sfl1 and Flo8 to the  FLO11 promoter.	bind
80302	1	3317	11	NULL	NULL	0	NULL	TS aceA	Protein		is					Transcriptional start site	NucleicAcidSubstance	aceA			NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_7_2554_s_206	16547043	(A) Transcriptional start sites of  aceA and  aceB are designated TS aceA and TS aceB, respectively, and the RamB binding site is designated the 13-bp motif.	bind
80303	2	3317	11	NULL	NULL	0	NULL	TS aceB	NucleicAcidSubstance		is					Transcriptional start sites	NucleicAcidSubstance	aceB			NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_7_2554_s_206	16547043	(A) Transcriptional start sites of  aceA and  aceB are designated TS aceA and TS aceB, respectively, and the RamB binding site is designated the 13-bp motif.	bind
80304	3	3317	11	NULL	NULL	0	NULL	RamB	Protein	binding site	is								13-bp motif		NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_7_2554_s_206	16547043	(A) Transcriptional start sites of  aceA and  aceB are designated TS aceA and TS aceB, respectively, and the RamB binding site is designated the 13-bp motif.	bind
8892	2	3318	5	11	NULL	0	NULL	SRP	Chemical		recognizes			10 hydrophobic residues		signal sequence	NucleicAcid	exposed sufficiently			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_24_6704_s_92	11118205	(A) translation of the polypeptide from the emergence of the tag sequence from the ribosome until the signal sequence is exposed sufficiently to be recognized by SRP ( 10 hydrophobic residues); (B) SRP binding to the nascent chain - ribosome complex; (C) targeting of the ternary complex to the ER membrane; and (D) translocation of the N-terminal portion across the membrane.	bind
8896	1	3318	5	11	NULL	0	NULL	polypeptide	AminoAcid	translation of	occurs					from ribosome	Cell	from emergence of the tag sequence			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_24_6704_s_92	11118205	(A) translation of the polypeptide from the emergence of the tag sequence from the ribosome until the signal sequence is exposed sufficiently to be recognized by SRP ( 10 hydrophobic residues); (B) SRP binding to the nascent chain - ribosome complex; (C) targeting of the ternary complex to the ER membrane; and (D) translocation of the N-terminal portion across the membrane.	bind
8898	3	3318	5	11	NULL	0	NULL	statement 1	Process		occurs untill					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_24_6704_s_92	11118205	(A) translation of the polypeptide from the emergence of the tag sequence from the ribosome until the signal sequence is exposed sufficiently to be recognized by SRP ( 10 hydrophobic residues); (B) SRP binding to the nascent chain - ribosome complex; (C) targeting of the ternary complex to the ER membrane; and (D) translocation of the N-terminal portion across the membrane.	bind
8899	4	3318	5	11	NULL	0	NULL	SRP	Chemical		bind					nascent chain - ribosome complex	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_24_6704_s_92	11118205	(A) translation of the polypeptide from the emergence of the tag sequence from the ribosome until the signal sequence is exposed sufficiently to be recognized by SRP ( 10 hydrophobic residues); (B) SRP binding to the nascent chain - ribosome complex; (C) targeting of the ternary complex to the ER membrane; and (D) translocation of the N-terminal portion across the membrane.	bind
8901	5	3318	5	11	NULL	0	NULL	ternary complex	GP		is targeted to					ER membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_24_6704_s_92	11118205	(A) translation of the polypeptide from the emergence of the tag sequence from the ribosome until the signal sequence is exposed sufficiently to be recognized by SRP ( 10 hydrophobic residues); (B) SRP binding to the nascent chain - ribosome complex; (C) targeting of the ternary complex to the ER membrane; and (D) translocation of the N-terminal portion across the membrane.	bind
8902	6	3318	5	11	NULL	0	NULL				is translocated across			N-terminal portion		membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_24_6704_s_92	11118205	(A) translation of the polypeptide from the emergence of the tag sequence from the ribosome until the signal sequence is exposed sufficiently to be recognized by SRP ( 10 hydrophobic residues); (B) SRP binding to the nascent chain - ribosome complex; (C) targeting of the ternary complex to the ER membrane; and (D) translocation of the N-terminal portion across the membrane.	bind
10349	1	3318	7	11	NULL	0	NULL	SRP	Chemical		bind					nascent chain - ribosome complex	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_24_6704_s_92	11118205	(A) translation of the polypeptide from the emergence of the tag sequence from the ribosome until the signal sequence is exposed sufficiently to be recognized by SRP ( 10 hydrophobic residues); (B) SRP binding to the nascent chain - ribosome complex; (C) targeting of the ternary complex to the ER membrane; and (D) translocation of the N-terminal portion across the membrane.	bind
10350	2	3318	7	11	NULL	0	NULL	ternary complex	GP		is targeted to					ER membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_24_6704_s_92	11118205	(A) translation of the polypeptide from the emergence of the tag sequence from the ribosome until the signal sequence is exposed sufficiently to be recognized by SRP ( 10 hydrophobic residues); (B) SRP binding to the nascent chain - ribosome complex; (C) targeting of the ternary complex to the ER membrane; and (D) translocation of the N-terminal portion across the membrane.	bind
10351	3	3318	7	11	NULL	0	NULL				translocates across the			N-terminal portion 		membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_24_6704_s_92	11118205	(A) translation of the polypeptide from the emergence of the tag sequence from the ribosome until the signal sequence is exposed sufficiently to be recognized by SRP ( 10 hydrophobic residues); (B) SRP binding to the nascent chain - ribosome complex; (C) targeting of the ternary complex to the ER membrane; and (D) translocation of the N-terminal portion across the membrane.	bind
14950	4	3318	7	11	NULL	0	NULL	SRP	Chemical		recognizes			10 hydrophobic residues		Signal sequence	NucleicAcid	sufficiently exposed			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_24_6704_s_92	11118205	(A) translation of the polypeptide from the emergence of the tag sequence from the ribosome until the signal sequence is exposed sufficiently to be recognized by SRP ( 10 hydrophobic residues); (B) SRP binding to the nascent chain - ribosome complex; (C) targeting of the ternary complex to the ER membrane; and (D) translocation of the N-terminal portion across the membrane.	bind
80305	1	3318	11	NULL	NULL	0	NULL	SRP	SmallMolecule		binds to 					ribosome complex	CellComponent	nascent chain			NULL		0	NULL	NULL	NULL	gw60_embo_19_24_6704_s_92	11118205	(A) translation of the polypeptide from the emergence of the tag sequence from the ribosome until the signal sequence is exposed sufficiently to be recognized by SRP ( 10 hydrophobic residues); (B) SRP binding to the nascent chain - ribosome complex; (C) targeting of the ternary complex to the ER membrane; and (D) translocation of the N-terminal portion across the membrane.	bind
80306	2	3318	11	NULL	NULL	0	NULL	ternary complex	PartOfProtein		targets to					ER membrane	CellComponent				NULL		0	NULL	NULL	NULL	gw60_embo_19_24_6704_s_92	11118205	(A) translation of the polypeptide from the emergence of the tag sequence from the ribosome until the signal sequence is exposed sufficiently to be recognized by SRP ( 10 hydrophobic residues); (B) SRP binding to the nascent chain - ribosome complex; (C) targeting of the ternary complex to the ER membrane; and (D) translocation of the N-terminal portion across the membrane.	bind
80338	3	3318	11	NULL	NULL	0	NULL	nascent chain	NucleicAcidSubstance		complex with 					ribosome complex	CellComponent				NULL		0	NULL	NULL	NULL	gw60_embo_19_24_6704_s_92	11118205	(A) translation of the polypeptide from the emergence of the tag sequence from the ribosome until the signal sequence is exposed sufficiently to be recognized by SRP ( 10 hydrophobic residues); (B) SRP binding to the nascent chain - ribosome complex; (C) targeting of the ternary complex to the ER membrane; and (D) translocation of the N-terminal portion across the membrane.	bind
80339	4	3318	11	NULL	NULL	0	NULL	SRP	SmallMolecule		binds to 					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_embo_19_24_6704_s_92	11118205	(A) translation of the polypeptide from the emergence of the tag sequence from the ribosome until the signal sequence is exposed sufficiently to be recognized by SRP ( 10 hydrophobic residues); (B) SRP binding to the nascent chain - ribosome complex; (C) targeting of the ternary complex to the ER membrane; and (D) translocation of the N-terminal portion across the membrane.	bind
80340	5	3318	11	NULL	NULL	0	NULL	ternary complex	Protein		targets to					ER membrane	CellComponent				NULL		0	NULL	NULL	NULL	gw60_embo_19_24_6704_s_92	11118205	(A) translation of the polypeptide from the emergence of the tag sequence from the ribosome until the signal sequence is exposed sufficiently to be recognized by SRP ( 10 hydrophobic residues); (B) SRP binding to the nascent chain - ribosome complex; (C) targeting of the ternary complex to the ER membrane; and (D) translocation of the N-terminal portion across the membrane.	bind
8422	1	3322	5	11	NULL	0	NULL	Ufd2	GP		bind					Cdc48	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_3_840_s_40	15240124	(A) Ufd2 binds with Cdc48.	bind
10352	1	3322	7	11	NULL	0	NULL	Ufd2	GP		binds					Cdc48	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_3_840_s_40	15240124	(A) Ufd2 binds with Cdc48.	bind
80341	1	3322	11	NULL	NULL	0	NULL	Ufd2	Protein		binds to 					Cdc48	Protein				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_3_840_s_40	15240124	(A) Ufd2 binds with Cdc48.	bind
8423	1	3323	5	11	NULL	0	NULL	RSK2	GP	unphosphorylated	bind					CBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_20_7089_s_114	11564891	(A) Unphosphorylated RSK2 binds to CBP. COS-1 cells were cotransfected with wild-type RSK2 and CBP and left untreated, treated with EGF, treated with EGF and PD98059, or cotransfected with PDK1.	bind
10353	1	3323	7	11	NULL	0	NULL	RSK2	GP	Unphosphorylated	binds to					CBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_20_7089_s_114	11564891	(A) Unphosphorylated RSK2 binds to CBP. COS-1 cells were cotransfected with wild-type RSK2 and CBP and left untreated, treated with EGF, treated with EGF and PD98059, or cotransfected with PDK1.	bind
80342	1	3323	11	NULL	NULL	0	NULL	RSK2	Protein	Unphosphorylated	binds to 					CBP	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_20_7089_s_114	11564891	(A) Unphosphorylated RSK2 binds to CBP. COS-1 cells were cotransfected with wild-type RSK2 and CBP and left untreated, treated with EGF, treated with EGF and PD98059, or cotransfected with PDK1.	bind
80343	2	3323	11	NULL	NULL	0	NULL	COS-1 cells	cell		transfected with					RSK2	Protein	wild-type			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_20_7089_s_114	11564891	(A) Unphosphorylated RSK2 binds to CBP. COS-1 cells were cotransfected with wild-type RSK2 and CBP and left untreated, treated with EGF, treated with EGF and PD98059, or cotransfected with PDK1.	bind
80344	3	3323	11	NULL	NULL	0	NULL	COS-1 cells	cell		transfected with					CBP	Protein	wild-type			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_20_7089_s_114	11564891	(A) Unphosphorylated RSK2 binds to CBP. COS-1 cells were cotransfected with wild-type RSK2 and CBP and left untreated, treated with EGF, treated with EGF and PD98059, or cotransfected with PDK1.	bind
80345	4	3323	11	NULL	NULL	0	NULL	statement 2	Process		occurs along with					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_20_7089_s_114	11564891	(A) Unphosphorylated RSK2 binds to CBP. COS-1 cells were cotransfected with wild-type RSK2 and CBP and left untreated, treated with EGF, treated with EGF and PD98059, or cotransfected with PDK1.	bind
80346	1	3324	11	NULL	NULL	0	NULL	PRE	CellComponent		is					preimmune serum	CellComponent				NULL		0	NULL	NULL	NULL	gw60_molcell_8_1_137_s_68	11511367	(A) Untreated interphase extract (Control), extract incubated with protein A beads bound to preimmune serum (PRE), and extract incubated with protein A beads bound to anti-X-Mre11 antibodies (X-Mre11 Ab) were probed with a polyclonal serum specific for X-Mre11 protein.	bind
80347	2	3324	11	NULL	NULL	0	NULL	extract	AnatomicalPart		incubated with					protein A	Protein	beads			NULL		0	NULL	NULL	NULL	gw60_molcell_8_1_137_s_68	11511367	(A) Untreated interphase extract (Control), extract incubated with protein A beads bound to preimmune serum (PRE), and extract incubated with protein A beads bound to anti-X-Mre11 antibodies (X-Mre11 Ab) were probed with a polyclonal serum specific for X-Mre11 protein.	bind
80348	3	3324	11	NULL	NULL	0	NULL	statement 2	AnatomicalPart		binds to 					preimmune serum	CellComponent				NULL		0	NULL	NULL	NULL	gw60_molcell_8_1_137_s_68	11511367	(A) Untreated interphase extract (Control), extract incubated with protein A beads bound to preimmune serum (PRE), and extract incubated with protein A beads bound to anti-X-Mre11 antibodies (X-Mre11 Ab) were probed with a polyclonal serum specific for X-Mre11 protein.	bind
80349	4	3324	11	NULL	NULL	0	NULL	statement 2	AnatomicalPart		binds to 					anti-X-Mre11 antibodies	Protein				NULL		0	NULL	NULL	NULL	gw60_molcell_8_1_137_s_68	11511367	(A) Untreated interphase extract (Control), extract incubated with protein A beads bound to preimmune serum (PRE), and extract incubated with protein A beads bound to anti-X-Mre11 antibodies (X-Mre11 Ab) were probed with a polyclonal serum specific for X-Mre11 protein.	bind
80350	5	3324	11	NULL	NULL	0	NULL	anti-X-Mre11 antibodies	Protein		is					X-Mre11 Ab	Protein				NULL		0	NULL	NULL	NULL	gw60_molcell_8_1_137_s_68	11511367	(A) Untreated interphase extract (Control), extract incubated with protein A beads bound to preimmune serum (PRE), and extract incubated with protein A beads bound to anti-X-Mre11 antibodies (X-Mre11 Ab) were probed with a polyclonal serum specific for X-Mre11 protein.	bind
8424	1	3325	5	11	NULL	0	NULL	Upc2p	GP		bind		directly			ERG2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6395_s_267	11533229	(A) Upc2p bound directly to the  ERG2 promoter in a SRE-dependent manner.	bind
8425	2	3325	5	11	NULL	0	NULL	statement 1	Process		is dependent on									SRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6395_s_267	11533229	(A) Upc2p bound directly to the  ERG2 promoter in a SRE-dependent manner.	bind
10354	1	3325	7	11	NULL	0	NULL	Upc2p	GP		bind		directly			ERG2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6395_s_267	11533229	(A) Upc2p bound directly to the  ERG2 promoter in a SRE-dependent manner.	bind
10355	2	3325	7	11	NULL	0	NULL	statement 1	Process		is dependent on					SRE	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6395_s_267	11533229	(A) Upc2p bound directly to the  ERG2 promoter in a SRE-dependent manner.	bind
80351	1	3325	11	NULL	NULL	0	NULL	Upc2p	Protein		binds to 		 directly			ERG2 promoter	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_19_6395_s_267	11533229	(A) Upc2p bound directly to the  ERG2 promoter in a SRE-dependent manner.	bind
80352	2	3325	11	NULL	NULL	0	NULL	statement 1	Process		depends on					SRE	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_19_6395_s_267	11533229	(A) Upc2p bound directly to the  ERG2 promoter in a SRE-dependent manner.	bind
8426	1	3329	5	11	NULL	0	NULL	Vimentin	GP		bind		preferentially			Fyn	GP		SH2 domain		NULL	in pervanadate-treated MC/9 mast cells	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_310_1_202_s_80	14511671	(A) Vimentin, pyruvate kinase, and SLP-76 in pervanadate-treated MC/9 mast cells  preferentially bound to the SH2 domain of Fyn.	bind
8427	2	3329	5	11	NULL	0	NULL	pyruvate kinase	GP		bind		preferentially			Fyn	GP		SH2 domain		NULL	in pervanadate-treated MC/9 mast cells	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_310_1_202_s_80	14511671	(A) Vimentin, pyruvate kinase, and SLP-76 in pervanadate-treated MC/9 mast cells  preferentially bound to the SH2 domain of Fyn.	bind
8428	3	3329	5	11	NULL	0	NULL	SLP-76	GP		bind		preferentially			Fyn	GP		SH2 domain		NULL	in pervanadate-treated MC/9 mast cells	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_310_1_202_s_80	14511671	(A) Vimentin, pyruvate kinase, and SLP-76 in pervanadate-treated MC/9 mast cells  preferentially bound to the SH2 domain of Fyn.	bind
10356	1	3329	7	11	NULL	0	NULL	Vimentin	GP		bind		preferentially			Fyn	GP		SH2 domain		NULL	pervanadate-treated MC/9 mast cells 	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_310_1_202_s_80	14511671	(A) Vimentin, pyruvate kinase, and SLP-76 in pervanadate-treated MC/9 mast cells  preferentially bound to the SH2 domain of Fyn.	bind
10357	2	3329	7	11	NULL	0	NULL	 pyruvate kinase	GP		bind		preferentially			Fyn	GP		SH2		NULL	pervanadate-treated MC/9 mast cells 	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_310_1_202_s_80	14511671	(A) Vimentin, pyruvate kinase, and SLP-76 in pervanadate-treated MC/9 mast cells  preferentially bound to the SH2 domain of Fyn.	bind
10358	3	3329	7	11	NULL	0	NULL	SLP-76 	GP		bind		preferentially			Fyn	GP		SH2		NULL	pervanadate-treated MC/9 mast cells 	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_310_1_202_s_80	14511671	(A) Vimentin, pyruvate kinase, and SLP-76 in pervanadate-treated MC/9 mast cells  preferentially bound to the SH2 domain of Fyn.	bind
80353	1	3329	11	NULL	NULL	0	NULL	Vimentin	Protein		binds to 		preferentially			Fyn	Protein		SH2 domain		NULL	pervanadate-treated MC/9 mast cells	0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_310_1_202_s_80	14511671	(A) Vimentin, pyruvate kinase, and SLP-76 in pervanadate-treated MC/9 mast cells  preferentially bound to the SH2 domain of Fyn.	bind
80354	2	3329	11	NULL	NULL	0	NULL	pyruvate kinase	Protein		binds to 		preferentially			Fyn	Protein		SH2 domain		NULL	pervanadate-treated MC/9 mast cells	0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_310_1_202_s_80	14511671	(A) Vimentin, pyruvate kinase, and SLP-76 in pervanadate-treated MC/9 mast cells  preferentially bound to the SH2 domain of Fyn.	bind
80355	3	3329	11	NULL	NULL	0	NULL	SLP-76	Protein		binds to 		preferentially			Fyn	Protein		SH2 domain		NULL	pervanadate-treated MC/9 mast cells	0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_310_1_202_s_80	14511671	(A) Vimentin, pyruvate kinase, and SLP-76 in pervanadate-treated MC/9 mast cells  preferentially bound to the SH2 domain of Fyn.	bind
8429	1	3330	5	11	NULL	0	NULL	Vps21p	GP		bind					Vac1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_3_159_s_65	10021387	(a) Vps21p binds Vac1p and Vps9p.	bind
8430	2	3330	5	11	NULL	0	NULL	Vps21p	GP		bind					Vps9p	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_3_159_s_65	10021387	(a) Vps21p binds Vac1p and Vps9p.	bind
10359	1	3330	7	11	NULL	0	NULL	Vps21p	GP		binds					Vac1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_3_159_s_65	10021387	(a) Vps21p binds Vac1p and Vps9p.	bind
10360	2	3330	7	11	NULL	0	NULL	Vps21p	GP		binds					Vps9p	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_3_159_s_65	10021387	(a) Vps21p binds Vac1p and Vps9p.	bind
80356	1	3330	11	NULL	NULL	0	NULL	Vps21p	Protein		binds to 					Vac1p	Protein				NULL		0	NULL	NULL	NULL	gw60_currbiol_9_3_159_s_65	10021387	(a) Vps21p binds Vac1p and Vps9p.	bind
80357	2	3330	11	NULL	NULL	0	NULL	Vps21p	Protein		binds to 					Vps9p	Protein				NULL		0	NULL	NULL	NULL	gw60_currbiol_9_3_159_s_65	10021387	(a) Vps21p binds Vac1p and Vps9p.	bind
8431	1	3333	5	11	NULL	0	NULL	cyclin A	GP		bind					p107 derivatives	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5380_s_292	9710622	(A) Western blot analysis of cyclin A bound to p107 derivatives.	bind
10361	1	3333	7	11	NULL	0	NULL	cyclin A	GP		bind					p107 derivatives	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5380_s_292	9710622	(A) Western blot analysis of cyclin A bound to p107 derivatives.	bind
80358	1	3333	11	NULL	NULL	0	NULL	cyclin A	Protein		binds to 					p107 derivative	Protein 				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_9_5380_s_292	9710622	(A) Western blot analysis of cyclin A bound to p107 derivatives.	bind
8432	1	3334	5	11	NULL	0	NULL	tn-R2 antibody	GP		bind					TN-R	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainres_863_1_42_s_83	10773191	(A) Western blot analysis of tn-R2 and 473 HD antibody binding to TN-R.	bind
8433	2	3334	5	11	NULL	0	NULL	473 HD antibody	GP		bind					TN-R	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainres_863_1_42_s_83	10773191	(A) Western blot analysis of tn-R2 and 473 HD antibody binding to TN-R.	bind
10362	1	3334	7	11	NULL	0	NULL	tn-R2 	GP		bind					TN-R	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainres_863_1_42_s_83	10773191	(A) Western blot analysis of tn-R2 and 473 HD antibody binding to TN-R.	bind
10363	2	3334	7	11	NULL	0	NULL	473 HD antibody 	GP		bind					TN-R	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainres_863_1_42_s_83	10773191	(A) Western blot analysis of tn-R2 and 473 HD antibody binding to TN-R.	bind
80359	1	3334	11	NULL	NULL	NULL	NULL	tn-R2 antibody	PartOfProtein		binds to 					TN-R	Protein				NULL		NULL	NULL	NULL	NULL	gw60_brainres_863_1_42_s_83	10773191	(A) Western blot analysis of tn-R2 and 473 HD antibody binding to TN-R.	bind
80360	2	3334	11	NULL	NULL	0	NULL	473 HD antibody 	PartOfProtein		binds to 					TN-R	Protein				NULL		0	NULL	NULL	NULL	gw60_brainres_863_1_42_s_83	10773191	(A) Western blot analysis of tn-R2 and 473 HD antibody binding to TN-R.	bind
8434	1	3335	5	11	NULL	0	NULL	6His-CD45	GP		bind			C817S		GST proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_40_s_221	12922168	(A) Western blot of 6His-CD45C817S (upper panel) or 6His-Lck SH2 (lower panel) remaining bound to GST proteins.	bind
8435	2	3335	5	11	NULL	0	NULL	6His-Lck	GP		bind			SH2		GST proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_40_s_221	12922168	(A) Western blot of 6His-CD45C817S (upper panel) or 6His-Lck SH2 (lower panel) remaining bound to GST proteins.	bind
10364	1	3335	7	11	NULL	0	NULL	6His-CD45 	GP		bind			C817S		GST protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_40_s_221	12922168	(A) Western blot of 6His-CD45C817S (upper panel) or 6His-Lck SH2 (lower panel) remaining bound to GST proteins.	bind
10365	2	3335	7	11	NULL	0	NULL	6His-Lck 	GP		bind			SH2 		GST protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_40_s_221	12922168	(A) Western blot of 6His-CD45C817S (upper panel) or 6His-Lck SH2 (lower panel) remaining bound to GST proteins.	bind
80361	1	3335	11	NULL	NULL	0	NULL	6His-CD45C817S	PartOfProtein		binds to 					GST proteins	Protein				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_40_s_221	12922168	(A) Western blot of 6His-CD45C817S (upper panel) or 6His-Lck SH2 (lower panel) remaining bound to GST proteins.	bind
80362	2	3335	11	NULL	NULL	0	NULL	6His-Lck SH2	PartOfProtein		binds to 					GST proteins	Protein				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_40_s_221	12922168	(A) Western blot of 6His-CD45C817S (upper panel) or 6His-Lck SH2 (lower panel) remaining bound to GST proteins.	bind
8436	1	3336	5	11	NULL	0	NULL	6His-Lck	GP		bind			SH2		GST proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_40_s_204	12922168	(A) Western blot of 6His-Lck SH2 remaining bound to various GST proteins (indicated above the blot) detected with an anti-6His antibody.	bind
11729	1	3336	7	11	NULL	0	NULL	 6His-Lck	GP		bind			SH2		GST protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_40_s_204	12922168	(A) Western blot of 6His-Lck SH2 remaining bound to various GST proteins (indicated above the blot) detected with an anti-6His antibody.	bind
80363	1	3336	11	NULL	NULL	0	NULL	6His-Lck SH2	PartOfProtein		binds to 					GST proteins	Protein				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_40_s_204	12922168	(A) Western blot of 6His-Lck SH2 remaining bound to various GST proteins (indicated above the blot) detected with an anti-6His antibody.	bind
80364	2	3336	11	NULL	NULL	0	NULL	statement 1	Process		detected with					anti-6His antibody	PartOfProtein				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_40_s_204	12922168	(A) Western blot of 6His-Lck SH2 remaining bound to various GST proteins (indicated above the blot) detected with an anti-6His antibody.	bind
8437	1	3337	5	11	NULL	0	NULL	JAS	Chemical		alter					actin	GP	distribution of			NULL	in T. gondii	NULL	NULL	NULL	NULL	gw60_molbiolcell_14_2_396_s_144	12589042	(A) Wide-field fluorescence microscopy demonstrates that JAS alters the distribution of actin in  T. gondii but does not affect microtubules (tubulin), reticular network filaments (IMC1), or myosin (TgMyoA tail).	bind
8438	2	3337	5	11	NULL	0	NULL	JAS	Chemical		does not affect					microtubules 	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_2_396_s_144	12589042	(A) Wide-field fluorescence microscopy demonstrates that JAS alters the distribution of actin in  T. gondii but does not affect microtubules (tubulin), reticular network filaments (IMC1), or myosin (TgMyoA tail).	bind
8439	3	3337	5	11	NULL	0	NULL	JAS	Chemical		does not affect					reticular network filaments	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_2_396_s_144	12589042	(A) Wide-field fluorescence microscopy demonstrates that JAS alters the distribution of actin in  T. gondii but does not affect microtubules (tubulin), reticular network filaments (IMC1), or myosin (TgMyoA tail).	bind
8440	4	3337	5	11	NULL	0	NULL	JAS	Chemical		did not affect					myosin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_2_396_s_144	12589042	(A) Wide-field fluorescence microscopy demonstrates that JAS alters the distribution of actin in  T. gondii but does not affect microtubules (tubulin), reticular network filaments (IMC1), or myosin (TgMyoA tail).	bind
54210	5	3337	5	11	NULL	0	NULL	microtubules	CellComponent		is					tubulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_2_396_s_144	12589042	(A) Wide-field fluorescence microscopy demonstrates that JAS alters the distribution of actin in  T. gondii but does not affect microtubules (tubulin), reticular network filaments (IMC1), or myosin (TgMyoA tail).	bind
54211	6	3337	5	11	NULL	0	NULL	IMC1	CellComponent		is					reticular network filaments	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_2_396_s_144	12589042	(A) Wide-field fluorescence microscopy demonstrates that JAS alters the distribution of actin in  T. gondii but does not affect microtubules (tubulin), reticular network filaments (IMC1), or myosin (TgMyoA tail).	bind
54212	7	3337	5	11	NULL	0	NULL	TgMyoA tail	GP		is					myosin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_2_396_s_144	12589042	(A) Wide-field fluorescence microscopy demonstrates that JAS alters the distribution of actin in  T. gondii but does not affect microtubules (tubulin), reticular network filaments (IMC1), or myosin (TgMyoA tail).	bind
10366	1	3337	7	11	NULL	0	NULL	JAS	Chemical		alters					actin	GP	distribution of			NULL	T. gondii 	NULL	NULL	NULL	NULL	gw60_molbiolcell_14_2_396_s_144	12589042	(A) Wide-field fluorescence microscopy demonstrates that JAS alters the distribution of actin in  T. gondii but does not affect microtubules (tubulin), reticular network filaments (IMC1), or myosin (TgMyoA tail).	bind
10367	2	3337	7	11	NULL	0	NULL	JAS	Chemical		does not affect					microtubules	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_2_396_s_144	12589042	(A) Wide-field fluorescence microscopy demonstrates that JAS alters the distribution of actin in  T. gondii but does not affect microtubules (tubulin), reticular network filaments (IMC1), or myosin (TgMyoA tail).	bind
10368	3	3337	7	11	NULL	0	NULL	JAS	Chemical		does not affect					 reticular network filaments 	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_2_396_s_144	12589042	(A) Wide-field fluorescence microscopy demonstrates that JAS alters the distribution of actin in  T. gondii but does not affect microtubules (tubulin), reticular network filaments (IMC1), or myosin (TgMyoA tail).	bind
10369	4	3337	7	11	NULL	0	NULL	JAS	Chemical		does not affect					myosin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_2_396_s_144	12589042	(A) Wide-field fluorescence microscopy demonstrates that JAS alters the distribution of actin in  T. gondii but does not affect microtubules (tubulin), reticular network filaments (IMC1), or myosin (TgMyoA tail).	bind
10370	5	3337	7	11	NULL	0	NULL	microtubule	CellComponent		is					tubulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_2_396_s_144	12589042	(A) Wide-field fluorescence microscopy demonstrates that JAS alters the distribution of actin in  T. gondii but does not affect microtubules (tubulin), reticular network filaments (IMC1), or myosin (TgMyoA tail).	bind
10371	6	3337	7	11	NULL	0	NULL	reticular network filaments 	CellComponent		is					IMCI	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_2_396_s_144	12589042	(A) Wide-field fluorescence microscopy demonstrates that JAS alters the distribution of actin in  T. gondii but does not affect microtubules (tubulin), reticular network filaments (IMC1), or myosin (TgMyoA tail).	bind
10372	7	3337	7	11	NULL	0	NULL	myosin	GP		is					TgMyoA tail	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_2_396_s_144	12589042	(A) Wide-field fluorescence microscopy demonstrates that JAS alters the distribution of actin in  T. gondii but does not affect microtubules (tubulin), reticular network filaments (IMC1), or myosin (TgMyoA tail).	bind
80365	1	3337	11	NULL	NULL	0	NULL	tubulin	CellComponent		is a type of 					microtubules	CellComponent				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_2_396_s_144	12589042	(A) Wide-field fluorescence microscopy demonstrates that JAS alters the distribution of actin in  T. gondii but does not affect microtubules (tubulin), reticular network filaments (IMC1), or myosin (TgMyoA tail).	bind
80366	2	3337	11	NULL	NULL	NULL	NULL	IMC1	CellComponent		is a type of 					reticular network filaments	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_2_396_s_144	12589042	(A) Wide-field fluorescence microscopy demonstrates that JAS alters the distribution of actin in  T. gondii but does not affect microtubules (tubulin), reticular network filaments (IMC1), or myosin (TgMyoA tail).	bind
80367	3	3337	11	NULL	NULL	0	NULL	TgMyoA	Protein		is a type of 					myosin	Protein				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_2_396_s_144	12589042	(A) Wide-field fluorescence microscopy demonstrates that JAS alters the distribution of actin in  T. gondii but does not affect microtubules (tubulin), reticular network filaments (IMC1), or myosin (TgMyoA tail).	bind
80368	4	3337	11	NULL	NULL	0	NULL	JAS	Chemical		alters		distribution of			actin	Protein	T. gondii			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_2_396_s_144	12589042	(A) Wide-field fluorescence microscopy demonstrates that JAS alters the distribution of actin in  T. gondii but does not affect microtubules (tubulin), reticular network filaments (IMC1), or myosin (TgMyoA tail).	bind
80369	5	3337	11	NULL	NULL	0	NULL	JAS	Chemical		does not affect					microtubules	CellComponent				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_2_396_s_144	12589042	(A) Wide-field fluorescence microscopy demonstrates that JAS alters the distribution of actin in  T. gondii but does not affect microtubules (tubulin), reticular network filaments (IMC1), or myosin (TgMyoA tail).	bind
80370	6	3337	11	NULL	NULL	0	NULL	JAS	Chemical		does not affect					reticular network filaments	CellComponent				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_2_396_s_144	12589042	(A) Wide-field fluorescence microscopy demonstrates that JAS alters the distribution of actin in  T. gondii but does not affect microtubules (tubulin), reticular network filaments (IMC1), or myosin (TgMyoA tail).	bind
80371	7	3337	11	NULL	NULL	0	NULL	JAS	Chemical		does not affect					myosin	CellComponent				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_2_396_s_144	12589042	(A) Wide-field fluorescence microscopy demonstrates that JAS alters the distribution of actin in  T. gondii but does not affect microtubules (tubulin), reticular network filaments (IMC1), or myosin (TgMyoA tail).	bind
80372	1	3338	11	NULL	NULL	0	NULL	Y79R ( )	PartOfProtein		is a type of 					actin binding mutant	PartOfProtein				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_211	11294914	(A) Wild-type ( ) and actin binding mutants Y79R ( ), K81E ( ), K81Y ( ), P107W ( ), P107Y ( ), A111E ( ), and minimally stable mutant C89S ( ).	bind
80373	2	3338	11	NULL	NULL	0	NULL	K81E ( )	PartOfProtein		is a type of 					actin binding mutant	PartOfProtein				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_211	11294914	(A) Wild-type ( ) and actin binding mutants Y79R ( ), K81E ( ), K81Y ( ), P107W ( ), P107Y ( ), A111E ( ), and minimally stable mutant C89S ( ).	bind
80374	3	3338	11	NULL	NULL	0	NULL	K81Y ( )	PartOfProtein		is a type of 					actin binding mutant	PartOfProtein				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_211	11294914	(A) Wild-type ( ) and actin binding mutants Y79R ( ), K81E ( ), K81Y ( ), P107W ( ), P107Y ( ), A111E ( ), and minimally stable mutant C89S ( ).	bind
80375	4	3338	11	NULL	NULL	0	NULL	P107W ( )	PartOfProtein		is a type of 					actin binding mutants	PartOfProtein				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_211	11294914	(A) Wild-type ( ) and actin binding mutants Y79R ( ), K81E ( ), K81Y ( ), P107W ( ), P107Y ( ), A111E ( ), and minimally stable mutant C89S ( ).	bind
80376	5	3338	11	NULL	NULL	0	NULL	P107Y ( )	PartOfProtein		is a type of 					actin binding mutant	PartOfProtein				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_211	11294914	(A) Wild-type ( ) and actin binding mutants Y79R ( ), K81E ( ), K81Y ( ), P107W ( ), P107Y ( ), A111E ( ), and minimally stable mutant C89S ( ).	bind
80377	6	3338	11	NULL	NULL	0	NULL	A111E ( )	PartOfProtein		is a type of 					actin binding mutant	PartOfProtein				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_4_1161_s_211	11294914	(A) Wild-type ( ) and actin binding mutants Y79R ( ), K81E ( ), K81Y ( ), P107W ( ), P107Y ( ), A111E ( ), and minimally stable mutant C89S ( ).	bind
8441	1	3339	5	11	NULL	0	NULL	s7betaCD	Chemical		bind					alphaHL	GP	WT			NULL		NULL	NULL	NULL	NULL	gw60_science_291_5504_636_s_32	11158673	(A) wild-type (WT), (B) M113N, and (C) N139Q alphaHL; ( D to  F) binding of s7betaCD to (D) WT, (E) M113N, and (F) N139Q alphaHL.	bind
8442	2	3339	5	11	NULL	0	NULL	s7betaCD	Chemical		bind					alphaHL	GP		M113N		NULL		NULL	NULL	NULL	NULL	gw60_science_291_5504_636_s_32	11158673	(A) wild-type (WT), (B) M113N, and (C) N139Q alphaHL; ( D to  F) binding of s7betaCD to (D) WT, (E) M113N, and (F) N139Q alphaHL.	bind
8443	3	3339	5	11	NULL	0	NULL	s7betaCD	Chemical		bind					alphaHL	GP		N139Q		NULL		NULL	NULL	NULL	NULL	gw60_science_291_5504_636_s_32	11158673	(A) wild-type (WT), (B) M113N, and (C) N139Q alphaHL; ( D to  F) binding of s7betaCD to (D) WT, (E) M113N, and (F) N139Q alphaHL.	bind
10373	1	3339	7	11	NULL	0	NULL	s7betaCD	Chemical		bind					alphaHL	GP	WT			NULL		NULL	NULL	NULL	NULL	gw60_science_291_5504_636_s_32	11158673	(A) wild-type (WT), (B) M113N, and (C) N139Q alphaHL; ( D to  F) binding of s7betaCD to (D) WT, (E) M113N, and (F) N139Q alphaHL.	bind
10374	2	3339	7	11	NULL	0	NULL	s7betaCD	Chemical		bind					alphaHL	GP		N139Q		NULL		NULL	NULL	NULL	NULL	gw60_science_291_5504_636_s_32	11158673	(A) wild-type (WT), (B) M113N, and (C) N139Q alphaHL; ( D to  F) binding of s7betaCD to (D) WT, (E) M113N, and (F) N139Q alphaHL.	bind
10375	3	3339	7	11	NULL	0	NULL	s7betaCD	Chemical		bind					alphaHL	GP		M113N		NULL		NULL	NULL	NULL	NULL	gw60_science_291_5504_636_s_32	11158673	(A) wild-type (WT), (B) M113N, and (C) N139Q alphaHL; ( D to  F) binding of s7betaCD to (D) WT, (E) M113N, and (F) N139Q alphaHL.	bind
8444	1	3342	5	11	NULL	0	NULL	Siah-1 protein	GP	wild-type	bind					DCC	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_724_s_171	9858595	(A) Wild-type and mutant Siah-1 proteins bind to DCC in vitro.	bind
8445	2	3342	5	11	NULL	0	NULL	Siah-1 protein	GP	mutant	bind					DCC	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_724_s_171	9858595	(A) Wild-type and mutant Siah-1 proteins bind to DCC in vitro.	bind
10376	1	3342	7	11	NULL	0	NULL	Siah-1 protein	GP	Wild-type 	bind					DCC	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_724_s_171	9858595	(A) Wild-type and mutant Siah-1 proteins bind to DCC in vitro.	bind
10377	2	3342	7	11	NULL	0	NULL	Siah-1 protein	GP	mutant	bind					DCC	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_724_s_171	9858595	(A) Wild-type and mutant Siah-1 proteins bind to DCC in vitro.	bind
80378	1	3342	11	NULL	NULL	NULL	NULL	Siah-1 protein	Protein	Wild-type	binds to 					DCC	Protein				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_724_s_171	9858595	(A) Wild-type and mutant Siah-1 proteins bind to DCC in vitro.	bind
80379	2	3342	11	NULL	NULL	0	NULL	Siah-1 protein	Protein	mutant	binds to 					DCC	Protein				NULL	in vitro	0	NULL	NULL	NULL	gw60_molcellbiol_19_1_724_s_171	9858595	(A) Wild-type and mutant Siah-1 proteins bind to DCC in vitro.	bind
8446	1	3343	5	11	NULL	0	NULL	MCAK	GP	wild-type	bind					MT lattice	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_169_3_391_s_108	15883193	(A) Wild-type MCAK binds MT lattice in the absence of ATP (left, lane 1).	bind
8447	2	3343	5	11	NULL	0	NULL	statement 1	Process		in the abscence of					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_169_3_391_s_108	15883193	(A) Wild-type MCAK binds MT lattice in the absence of ATP (left, lane 1).	bind
10378	1	3343	7	11	NULL	0	NULL	MCAK	GP	wild-type	binds					MT lattice	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_169_3_391_s_108	15883193	(A) Wild-type MCAK binds MT lattice in the absence of ATP (left, lane 1).	bind
10379	2	3343	7	11	NULL	0	NULL	statement 1	Process		occurs in the absence of					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_169_3_391_s_108	15883193	(A) Wild-type MCAK binds MT lattice in the absence of ATP (left, lane 1).	bind
80380	1	3343	11	NULL	NULL	0	NULL	MCAK	Protein	Wild-type	binds to 					MT lattice	CellComponent				NULL	in the absence of ATP	0	NULL	NULL	NULL	gw70_cellbiol_169_3_391_s_108	15883193	(A) Wild-type MCAK binds MT lattice in the absence of ATP (left, lane 1).	bind
80381	1	3345	11	NULL	NULL	0	NULL	eIF4G1	Protein	yeast	binds to 					Pab1p	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_51_s_179	9418852	(A) with reasonable affinity, we next investigated their ability to associate with the Pab1p-binding regions of yeast eIF4G1 and eIF4G2.	bind
80382	2	3345	11	NULL	NULL	0	NULL	eIF4G2	Protein	yeast	binds to 					Pab1p	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_51_s_179	9418852	(A) with reasonable affinity, we next investigated their ability to associate with the Pab1p-binding regions of yeast eIF4G1 and eIF4G2.	bind
8448	1	3346	5	11	NULL	0	NULL	PlexB	GP		bind					Rac1	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_1_39_s_86	11604137	(A) Within PlexB 3 region, PlexB binds to Rac1 and Rac2 but not to other Rho family GTPases.	bind
8449	2	3346	5	11	NULL	0	NULL	PlexB	GP		bind					Rac2	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_1_39_s_86	11604137	(A) Within PlexB 3 region, PlexB binds to Rac1 and Rac2 but not to other Rho family GTPases.	bind
8450	3	3346	5	11	NULL	0	NULL	PlexB	GP		does not bind					Rho family GTPases	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_1_39_s_86	11604137	(A) Within PlexB 3 region, PlexB binds to Rac1 and Rac2 but not to other Rho family GTPases.	bind
10380	1	3346	7	11	NULL	0	NULL	PlexB	GP		bind					Rac1	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_1_39_s_86	11604137	(A) Within PlexB 3 region, PlexB binds to Rac1 and Rac2 but not to other Rho family GTPases.	bind
10381	2	3346	7	11	NULL	0	NULL	PlexB	GP		bind					Rac2	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_1_39_s_86	11604137	(A) Within PlexB 3 region, PlexB binds to Rac1 and Rac2 but not to other Rho family GTPases.	bind
10382	3	3346	7	11	NULL	0	NULL	PlexB	GP		does not bind					Rho family GTPases	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_1_39_s_86	11604137	(A) Within PlexB 3 region, PlexB binds to Rac1 and Rac2 but not to other Rho family GTPases.	bind
80383	1	3346	11	NULL	NULL	0	NULL	PlexB	Protein		binds to 					Rac1	Protein				NULL		0	NULL	NULL	NULL	gw60_neuron_32_1_39_s_86	11604137	(A) Within PlexB 3 region, PlexB binds to Rac1 and Rac2 but not to other Rho family GTPases.	bind
80384	2	3346	11	NULL	NULL	0	NULL	PlexB	Protein		binds to 					Rac2	Protein				NULL		0	NULL	NULL	NULL	gw60_neuron_32_1_39_s_86	11604137	(A) Within PlexB 3 region, PlexB binds to Rac1 and Rac2 but not to other Rho family GTPases.	bind
80385	3	3346	11	NULL	NULL	0	NULL	Rac1	Protein		is a type of 					Rho family GTPase	Protein				NULL		0	NULL	NULL	NULL	gw60_neuron_32_1_39_s_86	11604137	(A) Within PlexB 3 region, PlexB binds to Rac1 and Rac2 but not to other Rho family GTPases.	bind
80386	4	3346	11	NULL	NULL	0	NULL	Rac2	Protein		is a type of 					Rho family GTPase	Protein				NULL		0	NULL	NULL	NULL	gw60_neuron_32_1_39_s_86	11604137	(A) Within PlexB 3 region, PlexB binds to Rac1 and Rac2 but not to other Rho family GTPases.	bind
8451	1	3347	5	11	NULL	0	NULL	PC4	Chemical		bind					DNA bubble substrates					NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_13_6084_s_207	15199162	(A) XPG protein enhances PC4 binding to DNA bubble substrates.	bind
8452	2	3347	5	11	NULL	0	NULL	XPG protein	GP		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_13_6084_s_207	15199162	(A) XPG protein enhances PC4 binding to DNA bubble substrates.	bind
10383	1	3347	7	11	NULL	0	NULL	PC4	Chemical		bind					DNA bubble substrates					NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_13_6084_s_207	15199162	(A) XPG protein enhances PC4 binding to DNA bubble substrates.	bind
10384	2	3347	7	11	NULL	0	NULL	 XPG protein	GP		enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_13_6084_s_207	15199162	(A) XPG protein enhances PC4 binding to DNA bubble substrates.	bind
80387	1	3347	11	NULL	NULL	0	NULL	PC4	Protein		binds to 					DNA bubble	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_13_6084_s_207	15199162	(A) XPG protein enhances PC4 binding to DNA bubble substrates.	bind
80388	2	3347	11	NULL	NULL	0	NULL	XPG protein	Protein		enhances					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_13_6084_s_207	15199162	(A) XPG protein enhances PC4 binding to DNA bubble substrates.	bind
8453	1	3348	5	11	NULL	0	NULL	eIF4A	GP	yeast	bind					eIF4G1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5557_s_237	10409745	(A) Yeast eIF4A binds to eIF4G1 and eIF4G2 in vitro.	bind
8454	2	3348	5	11	NULL	0	NULL	eIF4A	GP	yeast	bind					eIF4G2	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5557_s_237	10409745	(A) Yeast eIF4A binds to eIF4G1 and eIF4G2 in vitro.	bind
10394	1	3348	7	11	NULL	0	NULL	eIF4A	GP	yeast	bind					eIF4G1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5557_s_237	10409745	(A) Yeast eIF4A binds to eIF4G1 and eIF4G2 in vitro.	bind
10395	2	3348	7	11	NULL	0	NULL	eIF4A	GP	yeast	bind					eIF4G2	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5557_s_237	10409745	(A) Yeast eIF4A binds to eIF4G1 and eIF4G2 in vitro.	bind
80389	1	3348	11	NULL	NULL	0	NULL	eIF4A	Protein	yeast	binds to 					eIF4G1	Protein				NULL	in vitro	0	NULL	NULL	NULL	gw60_molcellbiol_19_8_5557_s_237	10409745	(A) Yeast eIF4A binds to eIF4G1 and eIF4G2 in vitro.	bind
80390	2	3348	11	NULL	NULL	0	NULL	eIF4A	Protein	yeast	binds to 					eIF4G2	Protein				NULL	in vitro	0	NULL	NULL	NULL	gw60_molcellbiol_19_8_5557_s_237	10409745	(A) Yeast eIF4A binds to eIF4G1 and eIF4G2 in vitro.	bind
8455	1	3349	5	11	NULL	0	NULL	PRA1	GP		bind					Piccolo	GP		zinc finger domains		NULL		NULL	NULL	NULL	NULL	gw60_neuron_25_1_203_s_161	10707984	(A) Yeast two-hybrid assay assessing binding of PRA1 and rab3A to the Piccolo (Pic-Zn2) and rabphilin-3A (Rabp-Zn) zinc finger domains.	bind
8456	2	3349	5	11	NULL	0	NULL	rab3A	GP		bind					Piccolo	GP		zinc finger domains		NULL		NULL	NULL	NULL	NULL	gw60_neuron_25_1_203_s_161	10707984	(A) Yeast two-hybrid assay assessing binding of PRA1 and rab3A to the Piccolo (Pic-Zn2) and rabphilin-3A (Rabp-Zn) zinc finger domains.	bind
8457	3	3349	5	11	NULL	0	NULL	rab3A	GP		bind					rabphilin-3A	GP		zinc finger domains		NULL		NULL	NULL	NULL	NULL	gw60_neuron_25_1_203_s_161	10707984	(A) Yeast two-hybrid assay assessing binding of PRA1 and rab3A to the Piccolo (Pic-Zn2) and rabphilin-3A (Rabp-Zn) zinc finger domains.	bind
8458	4	3349	5	11	NULL	0	NULL	PRA1	GP		bind					rabphilin-3A	GP		zinc finger domains		NULL		NULL	NULL	NULL	NULL	gw60_neuron_25_1_203_s_161	10707984	(A) Yeast two-hybrid assay assessing binding of PRA1 and rab3A to the Piccolo (Pic-Zn2) and rabphilin-3A (Rabp-Zn) zinc finger domains.	bind
54213	5	3349	5	11	NULL	0	NULL	Piccolo	GP		is					Pic-Zn2	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_25_1_203_s_161	10707984	(A) Yeast two-hybrid assay assessing binding of PRA1 and rab3A to the Piccolo (Pic-Zn2) and rabphilin-3A (Rabp-Zn) zinc finger domains.	bind
54214	6	3349	5	11	NULL	0	NULL	Rabp-Zn	GP		is					rabphilin-3A	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_25_1_203_s_161	10707984	(A) Yeast two-hybrid assay assessing binding of PRA1 and rab3A to the Piccolo (Pic-Zn2) and rabphilin-3A (Rabp-Zn) zinc finger domains.	bind
10396	1	3349	7	11	NULL	0	NULL	PRA1	GP		bind					Piccolo	GP		zinc finger domain		NULL		NULL	NULL	NULL	NULL	gw60_neuron_25_1_203_s_161	10707984	(A) Yeast two-hybrid assay assessing binding of PRA1 and rab3A to the Piccolo (Pic-Zn2) and rabphilin-3A (Rabp-Zn) zinc finger domains.	bind
10397	2	3349	7	11	NULL	0	NULL	PRA1	GP		bind					rabphilin-3A 	GP		zinc finger domain		NULL		NULL	NULL	NULL	NULL	gw60_neuron_25_1_203_s_161	10707984	(A) Yeast two-hybrid assay assessing binding of PRA1 and rab3A to the Piccolo (Pic-Zn2) and rabphilin-3A (Rabp-Zn) zinc finger domains.	bind
10398	3	3349	7	11	NULL	0	NULL	rab3A	GP		bind					Piccolo	GP		zinc finger domain		NULL		NULL	NULL	NULL	NULL	gw60_neuron_25_1_203_s_161	10707984	(A) Yeast two-hybrid assay assessing binding of PRA1 and rab3A to the Piccolo (Pic-Zn2) and rabphilin-3A (Rabp-Zn) zinc finger domains.	bind
10399	4	3349	7	11	NULL	0	NULL	rab3A	GP		bind					rabphilin-3A 	GP		zinc finger domain		NULL		NULL	NULL	NULL	NULL	gw60_neuron_25_1_203_s_161	10707984	(A) Yeast two-hybrid assay assessing binding of PRA1 and rab3A to the Piccolo (Pic-Zn2) and rabphilin-3A (Rabp-Zn) zinc finger domains.	bind
10402	5	3349	7	11	NULL	0	NULL	Piccolo	GP		is					Pic-Zn2	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_25_1_203_s_161	10707984	(A) Yeast two-hybrid assay assessing binding of PRA1 and rab3A to the Piccolo (Pic-Zn2) and rabphilin-3A (Rabp-Zn) zinc finger domains.	bind
10405	6	3349	7	11	NULL	0	NULL	rabphilin-3A 	GP		is					Rabp-Zn	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_25_1_203_s_161	10707984	(A) Yeast two-hybrid assay assessing binding of PRA1 and rab3A to the Piccolo (Pic-Zn2) and rabphilin-3A (Rabp-Zn) zinc finger domains.	bind
80391	1	3349	11	NULL	NULL	NULL	NULL	PRA1	Protein		binds to 					Piccolo	Protein		zinc finger domain		NULL	Yeast two-hybrid assay	NULL	NULL	NULL	NULL	gw60_neuron_25_1_203_s_161	10707984	(A) Yeast two-hybrid assay assessing binding of PRA1 and rab3A to the Piccolo (Pic-Zn2) and rabphilin-3A (Rabp-Zn) zinc finger domains.	bind
80392	2	3349	11	NULL	NULL	0	NULL	PRA1	Protein		binds to 					rabphilin-3A	Protein		zinc finger domain		NULL	Yeast two-hybrid assay	0	NULL	NULL	NULL	gw60_neuron_25_1_203_s_161	10707984	(A) Yeast two-hybrid assay assessing binding of PRA1 and rab3A to the Piccolo (Pic-Zn2) and rabphilin-3A (Rabp-Zn) zinc finger domains.	bind
80393	3	3349	11	NULL	NULL	0	NULL	rab3A	Protein		binds to 					Piccolo	Protein		zinc finger domain		NULL	Yeast two-hybrid assay	0	NULL	NULL	NULL	gw60_neuron_25_1_203_s_161	10707984	(A) Yeast two-hybrid assay assessing binding of PRA1 and rab3A to the Piccolo (Pic-Zn2) and rabphilin-3A (Rabp-Zn) zinc finger domains.	bind
80394	4	3349	11	NULL	NULL	0	NULL	rab3A	Protein		binds to 					rabphilin-3A	Protein		zinc finger domain		NULL	Yeast two-hybrid assay	0	NULL	NULL	NULL	gw60_neuron_25_1_203_s_161	10707984	(A) Yeast two-hybrid assay assessing binding of PRA1 and rab3A to the Piccolo (Pic-Zn2) and rabphilin-3A (Rabp-Zn) zinc finger domains.	bind
80395	5	3349	11	NULL	NULL	0	NULL	Pic-Zn2	Protein		is					Piccolo			zinc finger domain		NULL		0	NULL	NULL	NULL	gw60_neuron_25_1_203_s_161	10707984	(A) Yeast two-hybrid assay assessing binding of PRA1 and rab3A to the Piccolo (Pic-Zn2) and rabphilin-3A (Rabp-Zn) zinc finger domains.	bind
80396	6	3349	11	NULL	NULL	0	NULL	Rabp-Zn	Protein		is					 rabphilin-3A	Protein		zinc finger domain		NULL		0	NULL	NULL	NULL	gw60_neuron_25_1_203_s_161	10707984	(A) Yeast two-hybrid assay assessing binding of PRA1 and rab3A to the Piccolo (Pic-Zn2) and rabphilin-3A (Rabp-Zn) zinc finger domains.	bind
8459	1	3352	5	11	NULL	0	NULL	ZPC	GP		bind					ZP receptors	GP	sperm			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1469_3_197_s_876	11063883	(A) ZP proteins (most likely ZPC) bind to sperm ZP receptors, leading to aggregation and tyrosine (Y) phosphorylation.	bind
8460	2	3352	5	11	NULL	0	NULL	statement 1	Process		leads to					aggregation	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1469_3_197_s_876	11063883	(A) ZP proteins (most likely ZPC) bind to sperm ZP receptors, leading to aggregation and tyrosine (Y) phosphorylation.	bind
8461	3	3352	5	11	NULL	0	NULL	statement 1	Process		leads to					tyrosine	AminoAcid	phosphorylation of 			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1469_3_197_s_876	11063883	(A) ZP proteins (most likely ZPC) bind to sperm ZP receptors, leading to aggregation and tyrosine (Y) phosphorylation.	bind
10408	1	3352	7	11	NULL	0	NULL	ZPC	GP		bind					ZP receptors	GP	sperm			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1469_3_197_s_876	11063883	(A) ZP proteins (most likely ZPC) bind to sperm ZP receptors, leading to aggregation and tyrosine (Y) phosphorylation.	bind
10410	2	3352	7	11	NULL	0	NULL	statement 1	Process		leads to					aggregation	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1469_3_197_s_876	11063883	(A) ZP proteins (most likely ZPC) bind to sperm ZP receptors, leading to aggregation and tyrosine (Y) phosphorylation.	bind
10413	3	3352	7	11	NULL	0	NULL	statement 1	Process		leads to					tyrosine 	AminoAcid	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1469_3_197_s_876	11063883	(A) ZP proteins (most likely ZPC) bind to sperm ZP receptors, leading to aggregation and tyrosine (Y) phosphorylation.	bind
80397	1	3352	11	NULL	NULL	0	NULL	ZPC	Protein		is a type of 					ZP protein	Protein				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1469_3_197_s_876	11063883	(A) ZP proteins (most likely ZPC) bind to sperm ZP receptors, leading to aggregation and tyrosine (Y) phosphorylation.	bind
80398	2	3352	11	NULL	NULL	0	NULL	ZP protein	Protein		binds to 					ZP receptor	Protein	sperm			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1469_3_197_s_876	11063883	(A) ZP proteins (most likely ZPC) bind to sperm ZP receptors, leading to aggregation and tyrosine (Y) phosphorylation.	bind
80399	3	3352	11	NULL	NULL	0	NULL	tyrosine	AminoAcid		is					Y	AminoAcid				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1469_3_197_s_876	11063883	(A) ZP proteins (most likely ZPC) bind to sperm ZP receptors, leading to aggregation and tyrosine (Y) phosphorylation.	bind
80400	4	3352	11	NULL	NULL	0	NULL	statement 2	Process		leads to					aggregation	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1469_3_197_s_876	11063883	(A) ZP proteins (most likely ZPC) bind to sperm ZP receptors, leading to aggregation and tyrosine (Y) phosphorylation.	bind
80401	5	3352	11	NULL	NULL	0	NULL	statement 2	Process		leads to					phosphorylation	MolecularProcess	tyrosine			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1469_3_197_s_876	11063883	(A) ZP proteins (most likely ZPC) bind to sperm ZP receptors, leading to aggregation and tyrosine (Y) phosphorylation.	bind
8462	1	3353	5	11	NULL	0	NULL	[11,12-3H(N)] all- trans retinol	Chemical		bind					RFABG	GP				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_7_1222_s_162	10393207	(A) [11,12-3H(N)] all- trans retinol (0.2 muM) bound to RFABG or   of a 100-fold excess unlabeled heme.	bind
8463	2	3353	5	11	NULL	0	NULL	[11,12-3H(N)] all- trans retinol	Chemical		bind					heme	Chemical	unlabeled			NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_7_1222_s_162	10393207	(A) [11,12-3H(N)] all- trans retinol (0.2 muM) bound to RFABG or   of a 100-fold excess unlabeled heme.	bind
8465	3	3353	5	11	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_7_1222_s_162	10393207	(A) [11,12-3H(N)] all- trans retinol (0.2 muM) bound to RFABG or   of a 100-fold excess unlabeled heme.	bind
10420	1	3353	7	11	NULL	0	NULL	[11,12-3H(N)] all- trans retinol 	Chemical		bind					heme	Chemical	unlabeled			NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_7_1222_s_162	10393207	(A) [11,12-3H(N)] all- trans retinol (0.2 muM) bound to RFABG or   of a 100-fold excess unlabeled heme.	bind
10421	2	3353	7	11	NULL	0	NULL	[11,12-3H(N)] all- trans retinol 	Chemical		bind					RFABG	GP				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_7_1222_s_162	10393207	(A) [11,12-3H(N)] all- trans retinol (0.2 muM) bound to RFABG or   of a 100-fold excess unlabeled heme.	bind
80402	1	3353	11	NULL	NULL	0	NULL	[11,12-3H(N)] all- trans retinol	Chemical		binds to 					RFABG	Chemical				NULL		0	NULL	NULL	NULL	gw60_jlipidres_40_7_1222_s_162	10393207	(A) [11,12-3H(N)] all- trans retinol (0.2 muM) bound to RFABG or   of a 100-fold excess unlabeled heme.	bind
8464	1	3354	5	11	NULL	0	NULL	CGRP	GP	Human	bind					HEK293EBNA cell membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1539_1_131_s_72	11389975	(A) [125]Human CGRP binding to HEK293EBNA cell membranes was assayed.	bind
10422	1	3354	7	11	NULL	0	NULL	CGRP 	GP	Human	bind					HEK293EBNA cell membranes 	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1539_1_131_s_72	11389975	(A) [125]Human CGRP binding to HEK293EBNA cell membranes was assayed.	bind
80403	1	3354	11	NULL	NULL	0	NULL	CGRP	Protein	Human	binds to 					cell membrane	CellComponent	HEK293EBNA cell			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1539_1_131_s_72	11389975	(A) [125]Human CGRP binding to HEK293EBNA cell membranes was assayed.	bind
8466	1	3357	5	11	NULL	0	NULL	ARD-1	GP		bind					9 S RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_21_13823_s_112	9153239	(A)) in 10-fold excess ( lanes 7 and  8) or tRNA in 50-fold excess ( lane 9) did not prevent binding of ARD-1 to 9 S RNA, both of these RNAs reduced 9 S-specific binding of ARD-1 when added in still greater excess.	bind
10423	1	3357	7	11	NULL	0	NULL	ARD-1	GP		bind					9 S RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_21_13823_s_112	9153239	(A)) in 10-fold excess ( lanes 7 and  8) or tRNA in 50-fold excess ( lane 9) did not prevent binding of ARD-1 to 9 S RNA, both of these RNAs reduced 9 S-specific binding of ARD-1 when added in still greater excess.	bind
80404	1	3357	11	NULL	NULL	0	NULL	ARD-1	GeneOrProtein		binds to 					 9 S RNA	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_21_13823_s_112	9153239	(A)) in 10-fold excess ( lanes 7 and  8) or tRNA in 50-fold excess ( lane 9) did not prevent binding of ARD-1 to 9 S RNA, both of these RNAs reduced 9 S-specific binding of ARD-1 when added in still greater excess.	bind
8469	1	3358	5	11	NULL	0	NULL	TIAR	GP		bind					tumor necrosis factor alpha mRNA	NucleicAcid			AU-rich element	NULL	in macrophages	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6287_s_43	10938105	(A)+ RNA in the cytoplasmic foci known as stress granules ( 28), and it has been reported previously ( 22) that TIAR binds to the translational regulatory AU-rich element of tumor necrosis factor alpha mRNA in macrophages and may be involved in translational repression.	bind
8470	2	3358	5	11	NULL	0	NULL	statement 1	Process		involved in		may be			translational repression	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6287_s_43	10938105	(A)+ RNA in the cytoplasmic foci known as stress granules ( 28), and it has been reported previously ( 22) that TIAR binds to the translational regulatory AU-rich element of tumor necrosis factor alpha mRNA in macrophages and may be involved in translational repression.	bind
10424	1	3358	7	11	NULL	0	NULL	TIAR	GP		bind					tumor necrosis factor alpha mRNA	NucleicAcid			AU-rich element 	NULL	macrophages	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6287_s_43	10938105	(A)+ RNA in the cytoplasmic foci known as stress granules ( 28), and it has been reported previously ( 22) that TIAR binds to the translational regulatory AU-rich element of tumor necrosis factor alpha mRNA in macrophages and may be involved in translational repression.	bind
10425	2	3358	7	11	NULL	0	NULL	statement 1	Process		 involved in		may be			translational repression	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6287_s_43	10938105	(A)+ RNA in the cytoplasmic foci known as stress granules ( 28), and it has been reported previously ( 22) that TIAR binds to the translational regulatory AU-rich element of tumor necrosis factor alpha mRNA in macrophages and may be involved in translational repression.	bind
80405	1	3358	11	NULL	NULL	0	NULL	RNA	NucleicAcidSubstance	cytoplasmic foci	is a type of 					stress granule	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_17_6287_s_43	10938105	(A)+ RNA in the cytoplasmic foci known as stress granules ( 28), and it has been reported previously ( 22) that TIAR binds to the translational regulatory AU-rich element of tumor necrosis factor alpha mRNA in macrophages and may be involved in translational repression.	bind
80406	2	3358	11	NULL	NULL	0	NULL	TIAR	Protein		binds to 					tumor necrosis factor alpha mRNA	NucleicAcidSubstance	 macrophages		translational regulatory AU-rich element	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_17_6287_s_43	10938105	(A)+ RNA in the cytoplasmic foci known as stress granules ( 28), and it has been reported previously ( 22) that TIAR binds to the translational regulatory AU-rich element of tumor necrosis factor alpha mRNA in macrophages and may be involved in translational repression.	bind
80407	3	3358	11	NULL	NULL	0	NULL	statement 2	Process		involved in		may be			translational repression	MolecularProcess				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_17_6287_s_43	10938105	(A)+ RNA in the cytoplasmic foci known as stress granules ( 28), and it has been reported previously ( 22) that TIAR binds to the translational regulatory AU-rich element of tumor necrosis factor alpha mRNA in macrophages and may be involved in translational repression.	bind
10426	1	3360	7	NULL	NULL	0	NULL	 FBF-binding elements 	NULL	predicted	bind	NULL				FBF	NULL				NULL		0	NULL	NULL	NULL	gw70_genetics_168_1_147_s_291	15454534	(A)+ tail; brackets, regions tested for binding; gray boxes, predicted FBF-binding elements  ( e.g., a, FBE-a); only solid boxes bind FBF (see below).	bind
10427	2	3360	7	NULL	NULL	0	NULL	FBF-binding elements 	NULL		is	NULL				FBE	NULL				NULL		0	NULL	NULL	NULL	gw70_genetics_168_1_147_s_291	15454534	(A)+ tail; brackets, regions tested for binding; gray boxes, predicted FBF-binding elements  ( e.g., a, FBE-a); only solid boxes bind FBF (see below).	bind
8471	1	3361	5	11	NULL	0	NULL	Cbl	GP		does not bind					EGFR	GP	inactive			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_8981_s_354	15456872	(A),  while previous work has shown that Cbl and SETA/CIN85 do not bind to the inactive  receptor, but that EGFR activation leads to phosphorylation of the EGFR and the binding  of Cbl and SETA/CIN85, which results in SETA/CIN85, Cbl, and EGFR ubiquitination  and EGFR internalization (B).	bind
8472	2	3361	5	11	NULL	0	NULL	SETA/CIN85	GP		does not bind					EGFR	GP	inactive			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_8981_s_354	15456872	(A),  while previous work has shown that Cbl and SETA/CIN85 do not bind to the inactive  receptor, but that EGFR activation leads to phosphorylation of the EGFR and the binding  of Cbl and SETA/CIN85, which results in SETA/CIN85, Cbl, and EGFR ubiquitination  and EGFR internalization (B).	bind
8473	3	3361	5	11	NULL	0	NULL	EGFR	GP	activation	leads to					EGFR	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_8981_s_354	15456872	(A),  while previous work has shown that Cbl and SETA/CIN85 do not bind to the inactive  receptor, but that EGFR activation leads to phosphorylation of the EGFR and the binding  of Cbl and SETA/CIN85, which results in SETA/CIN85, Cbl, and EGFR ubiquitination  and EGFR internalization (B).	bind
8474	4	3361	5	11	NULL	0	NULL	Cbl	GP		bind					SETA/CIN85	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_8981_s_354	15456872	(A),  while previous work has shown that Cbl and SETA/CIN85 do not bind to the inactive  receptor, but that EGFR activation leads to phosphorylation of the EGFR and the binding  of Cbl and SETA/CIN85, which results in SETA/CIN85, Cbl, and EGFR ubiquitination  and EGFR internalization (B).	bind
8476	5	3361	5	11	NULL	0	NULL	statement 4	Process		results in					SETA/CIN85	GP	ubiquitination of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_8981_s_354	15456872	(A),  while previous work has shown that Cbl and SETA/CIN85 do not bind to the inactive  receptor, but that EGFR activation leads to phosphorylation of the EGFR and the binding  of Cbl and SETA/CIN85, which results in SETA/CIN85, Cbl, and EGFR ubiquitination  and EGFR internalization (B).	bind
8478	6	3361	5	11	NULL	0	NULL	statement 4	Process		results in					Cbl	GP	ubiquitination of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_8981_s_354	15456872	(A),  while previous work has shown that Cbl and SETA/CIN85 do not bind to the inactive  receptor, but that EGFR activation leads to phosphorylation of the EGFR and the binding  of Cbl and SETA/CIN85, which results in SETA/CIN85, Cbl, and EGFR ubiquitination  and EGFR internalization (B).	bind
8480	7	3361	5	11	NULL	0	NULL	statement 4	Process		results in					EGFR	GP	ubiquitination of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_8981_s_354	15456872	(A),  while previous work has shown that Cbl and SETA/CIN85 do not bind to the inactive  receptor, but that EGFR activation leads to phosphorylation of the EGFR and the binding  of Cbl and SETA/CIN85, which results in SETA/CIN85, Cbl, and EGFR ubiquitination  and EGFR internalization (B).	bind
8482	8	3361	5	11	NULL	0	NULL	statement 4	Process		results in					EGFR	GP	internalization of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_8981_s_354	15456872	(A),  while previous work has shown that Cbl and SETA/CIN85 do not bind to the inactive  receptor, but that EGFR activation leads to phosphorylation of the EGFR and the binding  of Cbl and SETA/CIN85, which results in SETA/CIN85, Cbl, and EGFR ubiquitination  and EGFR internalization (B).	bind
10428	1	3361	7	11	NULL	0	NULL	Cbl	GP		does not bind					EGFR	GP	inactive			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_8981_s_354	15456872	(A),  while previous work has shown that Cbl and SETA/CIN85 do not bind to the inactive  receptor, but that EGFR activation leads to phosphorylation of the EGFR and the binding  of Cbl and SETA/CIN85, which results in SETA/CIN85, Cbl, and EGFR ubiquitination  and EGFR internalization (B).	bind
10429	2	3361	7	11	NULL	0	NULL	SETA/CIN85 	GP		does not bind					EGFR	GP	inactive			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_8981_s_354	15456872	(A),  while previous work has shown that Cbl and SETA/CIN85 do not bind to the inactive  receptor, but that EGFR activation leads to phosphorylation of the EGFR and the binding  of Cbl and SETA/CIN85, which results in SETA/CIN85, Cbl, and EGFR ubiquitination  and EGFR internalization (B).	bind
10430	3	3361	7	11	NULL	0	NULL	EGFR	GP	activated	leads to					EGFR	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_8981_s_354	15456872	(A),  while previous work has shown that Cbl and SETA/CIN85 do not bind to the inactive  receptor, but that EGFR activation leads to phosphorylation of the EGFR and the binding  of Cbl and SETA/CIN85, which results in SETA/CIN85, Cbl, and EGFR ubiquitination  and EGFR internalization (B).	bind
10431	4	3361	7	11	NULL	0	NULL	Cbl	GP		bind					SETA/CIN85	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_8981_s_354	15456872	(A),  while previous work has shown that Cbl and SETA/CIN85 do not bind to the inactive  receptor, but that EGFR activation leads to phosphorylation of the EGFR and the binding  of Cbl and SETA/CIN85, which results in SETA/CIN85, Cbl, and EGFR ubiquitination  and EGFR internalization (B).	bind
10432	5	3361	7	11	NULL	0	NULL	statement 4	Process		results in					SETA/CIN85	GP	ubiquitination of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_8981_s_354	15456872	(A),  while previous work has shown that Cbl and SETA/CIN85 do not bind to the inactive  receptor, but that EGFR activation leads to phosphorylation of the EGFR and the binding  of Cbl and SETA/CIN85, which results in SETA/CIN85, Cbl, and EGFR ubiquitination  and EGFR internalization (B).	bind
10433	6	3361	7	11	NULL	0	NULL	statement 4	Process		results in					Cbl	GP	ubiquitination of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_8981_s_354	15456872	(A),  while previous work has shown that Cbl and SETA/CIN85 do not bind to the inactive  receptor, but that EGFR activation leads to phosphorylation of the EGFR and the binding  of Cbl and SETA/CIN85, which results in SETA/CIN85, Cbl, and EGFR ubiquitination  and EGFR internalization (B).	bind
10434	7	3361	7	11	NULL	0	NULL	statement 4	Process		results in					EGFR	GP	ubiquitination of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_8981_s_354	15456872	(A),  while previous work has shown that Cbl and SETA/CIN85 do not bind to the inactive  receptor, but that EGFR activation leads to phosphorylation of the EGFR and the binding  of Cbl and SETA/CIN85, which results in SETA/CIN85, Cbl, and EGFR ubiquitination  and EGFR internalization (B).	bind
10435	8	3361	7	11	NULL	0	NULL	statement 4	Process		results in					EGFR	GP	internalization of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_8981_s_354	15456872	(A),  while previous work has shown that Cbl and SETA/CIN85 do not bind to the inactive  receptor, but that EGFR activation leads to phosphorylation of the EGFR and the binding  of Cbl and SETA/CIN85, which results in SETA/CIN85, Cbl, and EGFR ubiquitination  and EGFR internalization (B).	bind
80408	1	3361	11	NULL	NULL	0	NULL	Cbl	Protein		does not bind to					inactive receptor	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_20_8981_s_354	15456872	(A),  while previous work has shown that Cbl and SETA/CIN85 do not bind to the inactive  receptor, but that EGFR activation leads to phosphorylation of the EGFR and the binding  of Cbl and SETA/CIN85, which results in SETA/CIN85, Cbl, and EGFR ubiquitination  and EGFR internalization (B).	bind
80409	2	3361	11	NULL	NULL	0	NULL	SETA/CIN85	Protein		does not bind to					inactive receptor	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_20_8981_s_354	15456872	(A),  while previous work has shown that Cbl and SETA/CIN85 do not bind to the inactive  receptor, but that EGFR activation leads to phosphorylation of the EGFR and the binding  of Cbl and SETA/CIN85, which results in SETA/CIN85, Cbl, and EGFR ubiquitination  and EGFR internalization (B).	bind
80410	3	3361	11	NULL	NULL	0	NULL	EGFR	Protein	active	phosphorylate					EGFR	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_20_8981_s_354	15456872	(A),  while previous work has shown that Cbl and SETA/CIN85 do not bind to the inactive  receptor, but that EGFR activation leads to phosphorylation of the EGFR and the binding  of Cbl and SETA/CIN85, which results in SETA/CIN85, Cbl, and EGFR ubiquitination  and EGFR internalization (B).	bind
80411	4	3361	11	NULL	NULL	0	NULL	EGFR	Protein	active	binds to 					Cbl	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_20_8981_s_354	15456872	(A),  while previous work has shown that Cbl and SETA/CIN85 do not bind to the inactive  receptor, but that EGFR activation leads to phosphorylation of the EGFR and the binding  of Cbl and SETA/CIN85, which results in SETA/CIN85, Cbl, and EGFR ubiquitination  and EGFR internalization (B).	bind
80412	5	3361	11	NULL	NULL	0	NULL	EGFR	Protein	active	binds to 					SETA/CIN85	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_20_8981_s_354	15456872	(A),  while previous work has shown that Cbl and SETA/CIN85 do not bind to the inactive  receptor, but that EGFR activation leads to phosphorylation of the EGFR and the binding  of Cbl and SETA/CIN85, which results in SETA/CIN85, Cbl, and EGFR ubiquitination  and EGFR internalization (B).	bind
80413	6	3361	11	NULL	NULL	0	NULL	statement 3	Process		ubiquitinated					EGFR	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_20_8981_s_354	15456872	(A),  while previous work has shown that Cbl and SETA/CIN85 do not bind to the inactive  receptor, but that EGFR activation leads to phosphorylation of the EGFR and the binding  of Cbl and SETA/CIN85, which results in SETA/CIN85, Cbl, and EGFR ubiquitination  and EGFR internalization (B).	bind
80414	7	3361	11	NULL	NULL	0	NULL	statement 3	Process		internalize 					EGFR	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_20_8981_s_354	15456872	(A),  while previous work has shown that Cbl and SETA/CIN85 do not bind to the inactive  receptor, but that EGFR activation leads to phosphorylation of the EGFR and the binding  of Cbl and SETA/CIN85, which results in SETA/CIN85, Cbl, and EGFR ubiquitination  and EGFR internalization (B).	bind
80415	8	3361	11	NULL	NULL	0	NULL	statement 6	Process		occurs along with					statement 7	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_20_8981_s_354	15456872	(A),  while previous work has shown that Cbl and SETA/CIN85 do not bind to the inactive  receptor, but that EGFR activation leads to phosphorylation of the EGFR and the binding  of Cbl and SETA/CIN85, which results in SETA/CIN85, Cbl, and EGFR ubiquitination  and EGFR internalization (B).	bind
80416	9	3361	11	NULL	NULL	0	NULL	statement 4	Process		ubiquitinated					Cbl	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_20_8981_s_354	15456872	(A),  while previous work has shown that Cbl and SETA/CIN85 do not bind to the inactive  receptor, but that EGFR activation leads to phosphorylation of the EGFR and the binding  of Cbl and SETA/CIN85, which results in SETA/CIN85, Cbl, and EGFR ubiquitination  and EGFR internalization (B).	bind
80417	10	3361	11	NULL	NULL	0	NULL	statement 5	Process		ubiquitinated					SETA/CIN85	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_20_8981_s_354	15456872	(A),  while previous work has shown that Cbl and SETA/CIN85 do not bind to the inactive  receptor, but that EGFR activation leads to phosphorylation of the EGFR and the binding  of Cbl and SETA/CIN85, which results in SETA/CIN85, Cbl, and EGFR ubiquitination  and EGFR internalization (B).	bind
8484	1	3362	5	11	NULL	0	NULL	PT	Chemical		bind		covalently						alphaL262C		NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_307_1_42_s_247	14500778	(A), after propanethiol (PT) covalent binding to alphaL262C (B), and after PT covalent binding to alphaL263C (C).	bind
8485	2	3362	5	11	NULL	0	NULL	PT	Chemical		is					propanethiol	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_307_1_42_s_247	14500778	(A), after propanethiol (PT) covalent binding to alphaL262C (B), and after PT covalent binding to alphaL263C (C).	bind
8486	3	3362	5	11	NULL	0	NULL	PT	Chemical		bind		covalently						alphaL263C		NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_307_1_42_s_247	14500778	(A), after propanethiol (PT) covalent binding to alphaL262C (B), and after PT covalent binding to alphaL263C (C).	bind
10437	1	3362	7	11	NULL	0	NULL	propanethiol	Chemical		bind		covalently			alphaL262C	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_307_1_42_s_247	14500778	(A), after propanethiol (PT) covalent binding to alphaL262C (B), and after PT covalent binding to alphaL263C (C).	bind
10438	2	3362	7	11	NULL	0	NULL	propanethiol	Chemical		bind		covalently			alphaL263C	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_307_1_42_s_247	14500778	(A), after propanethiol (PT) covalent binding to alphaL262C (B), and after PT covalent binding to alphaL263C (C).	bind
10439	3	3362	7	11	NULL	0	NULL	propanethiol 	Chemical		is					PT	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_307_1_42_s_247	14500778	(A), after propanethiol (PT) covalent binding to alphaL262C (B), and after PT covalent binding to alphaL263C (C).	bind
80418	1	3362	11	NULL	NULL	0	NULL	propanethiol	Chemical		is					PT	Chemical				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_307_1_42_s_247	14500778	(A), after propanethiol (PT) covalent binding to alphaL262C (B), and after PT covalent binding to alphaL263C (C).	bind
80419	2	3362	11	NULL	NULL	0	NULL	propanethiol	Chemical		binds to 		covalent			alphaL262C	AminoAcid				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_307_1_42_s_247	14500778	(A), after propanethiol (PT) covalent binding to alphaL262C (B), and after PT covalent binding to alphaL263C (C).	bind
80420	3	3362	11	NULL	NULL	0	NULL	PT	Chemical		binds to 		covalent			alphaL263C	AminoAcid				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_307_1_42_s_247	14500778	(A), after propanethiol (PT) covalent binding to alphaL262C (B), and after PT covalent binding to alphaL263C (C).	bind
8487	1	3363	5	11	NULL	0	NULL	A2A 	GP		bind					hippocampal nerve terminals	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_301_2_441_s_156	11961042	(A), and A2A (B) adenosine receptors antibody binding to hippocampal nerve terminals.	bind
44757	2	3363	5	11	NULL	0	NULL	A2A	GP		is a type of					adenosine receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_301_2_441_s_156	11961042	(A), and A2A (B) adenosine receptors antibody binding to hippocampal nerve terminals.	bind
10440	1	3363	7	11	NULL	0	NULL	A2A	GP		bind					hippocampal nerve terminals	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_301_2_441_s_156	11961042	(A), and A2A (B) adenosine receptors antibody binding to hippocampal nerve terminals.	bind
44758	2	3363	7	11	NULL	0	NULL	A2A	GP		is a type of					adenosine receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_301_2_441_s_156	11961042	(A), and A2A (B) adenosine receptors antibody binding to hippocampal nerve terminals.	bind
80421	1	3363	11	NULL	NULL	0	NULL	A2A	Protein		is a type of 					adenosine receptor	Protein				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_301_2_441_s_156	11961042	(A), and A2A (B) adenosine receptors antibody binding to hippocampal nerve terminals.	bind
80422	2	3363	11	NULL	NULL	0	NULL	A2A	Protein	antibody	binds to 					nerve terminal	Organism part	hippocampal			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_301_2_441_s_156	11961042	(A), and A2A (B) adenosine receptors antibody binding to hippocampal nerve terminals.	bind
8488	1	3365	5	11	NULL	0	NULL	spectrin	GP	brain	bind					red blood cell membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1611_1_115_s_89	12659952	(A), binding of  the brain spectrin by red blood cell membranes (B), binding of the erythrocyte spectrin  by red blood cell membranes (C), and binding of the erythrocyte spectrin by synaptic  plasma membranes (D).	bind
8489	2	3365	5	11	NULL	0	NULL	spectrin	GP	erythrocyte	bind					red blood cell membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1611_1_115_s_89	12659952	(A), binding of  the brain spectrin by red blood cell membranes (B), binding of the erythrocyte spectrin  by red blood cell membranes (C), and binding of the erythrocyte spectrin by synaptic  plasma membranes (D).	bind
8490	3	3365	5	11	NULL	0	NULL	spectrin	GP	erythrocyte	bind					synaptic plasma membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1611_1_115_s_89	12659952	(A), binding of  the brain spectrin by red blood cell membranes (B), binding of the erythrocyte spectrin  by red blood cell membranes (C), and binding of the erythrocyte spectrin by synaptic  plasma membranes (D).	bind
10441	1	3365	7	11	NULL	0	NULL	spectrin	GP	brain	bind					red blood cell membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1611_1_115_s_89	12659952	(A), binding of  the brain spectrin by red blood cell membranes (B), binding of the erythrocyte spectrin  by red blood cell membranes (C), and binding of the erythrocyte spectrin by synaptic  plasma membranes (D).	bind
10442	2	3365	7	11	NULL	0	NULL	spectrin	GP	erythrocyte	bind					red blood cell membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1611_1_115_s_89	12659952	(A), binding of  the brain spectrin by red blood cell membranes (B), binding of the erythrocyte spectrin  by red blood cell membranes (C), and binding of the erythrocyte spectrin by synaptic  plasma membranes (D).	bind
10443	3	3365	7	11	NULL	0	NULL	spectrin	GP	erythrocyte	bind					synaptic plasma membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1611_1_115_s_89	12659952	(A), binding of  the brain spectrin by red blood cell membranes (B), binding of the erythrocyte spectrin  by red blood cell membranes (C), and binding of the erythrocyte spectrin by synaptic  plasma membranes (D).	bind
80423	1	3365	11	NULL	NULL	0	NULL	spectrin	Protein	brain	binds to 					cell membrane	CellComponent	red blood cell			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1611_1_115_s_89	12659952	(A), binding of  the brain spectrin by red blood cell membranes (B), binding of the erythrocyte spectrin  by red blood cell membranes (C), and binding of the erythrocyte spectrin by synaptic  plasma membranes (D).	bind
80424	2	3365	11	NULL	NULL	0	NULL	spectrin	Protein	erythrocyte	binds to 					cell membrane	CellComponent	red blood cell			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1611_1_115_s_89	12659952	(A), binding of  the brain spectrin by red blood cell membranes (B), binding of the erythrocyte spectrin  by red blood cell membranes (C), and binding of the erythrocyte spectrin by synaptic  plasma membranes (D).	bind
80425	3	3365	11	NULL	NULL	0	NULL	spectrin	Protein	erythrocyte	binds to 					plasma membrane	CellComponent	synaptic 			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1611_1_115_s_89	12659952	(A), binding of  the brain spectrin by red blood cell membranes (B), binding of the erythrocyte spectrin  by red blood cell membranes (C), and binding of the erythrocyte spectrin by synaptic  plasma membranes (D).	bind
8491	1	3366	5	11	NULL	0	NULL	spectrin	GP	brain	bind					red blood cell membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1611_1_115_s_89	12659952	(A), binding of the brain spectrin by red blood cell membranes (B), binding of the erythrocyte spectrin by red blood cell membranes (C), and binding of the erythrocyte spectrin by synaptic plasma membranes (D).	bind
8492	2	3366	5	11	NULL	0	NULL	spectrin	GP	erythrocyte	bind					red blood cell membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1611_1_115_s_89	12659952	(A), binding of the brain spectrin by red blood cell membranes (B), binding of the erythrocyte spectrin by red blood cell membranes (C), and binding of the erythrocyte spectrin by synaptic plasma membranes (D).	bind
8493	3	3366	5	11	NULL	0	NULL	spectrin	GP	erythrocyte	bind					synaptic plasma membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1611_1_115_s_89	12659952	(A), binding of the brain spectrin by red blood cell membranes (B), binding of the erythrocyte spectrin by red blood cell membranes (C), and binding of the erythrocyte spectrin by synaptic plasma membranes (D).	bind
8494	1	3367	5	11	NULL	0	NULL	Nef	GP		downregulate					CD4	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_70_2_548_s_73	16760313	(A), CD4 downregulation by Nef (B), and AP binding mediated by the Nef dileucine  motif (C).	bind
8495	2	3367	5	11	NULL	0	NULL	Nef	GP		mediate			dileucine motif		AP	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_70_2_548_s_73	16760313	(A), CD4 downregulation by Nef (B), and AP binding mediated by the Nef dileucine  motif (C).	bind
10444	1	3367	7	11	NULL	0	NULL	Nef	GP		downregulates					CD4	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_70_2_548_s_73	16760313	(A), CD4 downregulation by Nef (B), and AP binding mediated by the Nef dileucine  motif (C).	bind
10445	2	3367	7	11	NULL	0	NULL	Nef	GP		mediates			dileucine motif 		AP	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_70_2_548_s_73	16760313	(A), CD4 downregulation by Nef (B), and AP binding mediated by the Nef dileucine  motif (C).	bind
80426	1	3367	11	NULL	NULL	NULL	NULL	Nef	Protein		downregulate			dileucine motif		CD4	Protein				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_70_2_548_s_73	16760313	(A), CD4 downregulation by Nef (B), and AP binding mediated by the Nef dileucine  motif (C).	bind
80431	2	3367	11	NULL	NULL	0	NULL	AP	Protein		binds to 					CD4	Protein				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_70_2_548_s_73	16760313	(A), CD4 downregulation by Nef (B), and AP binding mediated by the Nef dileucine  motif (C).	bind
80432	3	3367	11	NULL	NULL	0	NULL	statement 2	Process		downregulate					CD4	Protein				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_70_2_548_s_73	16760313	(A), CD4 downregulation by Nef (B), and AP binding mediated by the Nef dileucine  motif (C).	bind
80434	4	3367	11	NULL	NULL	0	NULL	statement 3	Process		mediated by					Nef	Protein		dileucine motif 		NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_70_2_548_s_73	16760313	(A), CD4 downregulation by Nef (B), and AP binding mediated by the Nef dileucine  motif (C).	bind
8496	1	3368	5	11	NULL	0	NULL	Swi6p	GP		bind					CLN2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_9_3126_s_274	12697814	(A), cell size (B), expression of the  SCB: lacZ reporter gene (C), and binding of Swi6p to the  CLN2 promoter (D) were analyzed as described previously.	bind
10446	1	3368	7	11	NULL	0	NULL	Swi6p	GP		bind					CLN2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_9_3126_s_274	12697814	(A), cell size (B), expression of the  SCB: lacZ reporter gene (C), and binding of Swi6p to the  CLN2 promoter (D) were analyzed as described previously.	bind
80435	1	3368	11	NULL	NULL	0	NULL	Swi6p	Protein		binds to 					CLN2 promoter	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_9_3126_s_274	12697814	(A), cell size (B), expression of the  SCB: lacZ reporter gene (C), and binding of Swi6p to the  CLN2 promoter (D) were analyzed as described previously.	bind
8497	1	3369	5	11	NULL	0	NULL	delta50HA	GP		bind					X chromosome	Chromosome				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_20_8913_s_166	16199870	(A), delta50HA binds weakly (B), and delta26HA binds more strongly to the X chromosome than delta50HA (C); but staining intensity is consistently less than for MSL1NHA (Fig.  2C and D).	bind
8498	2	3369	5	11	NULL	0	NULL	delta26HA	GP		bind					X chromosome	Chromosome				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_20_8913_s_166	16199870	(A), delta50HA binds weakly (B), and delta26HA binds more strongly to the X chromosome than delta50HA (C); but staining intensity is consistently less than for MSL1NHA (Fig.  2C and D).	bind
8499	3	3369	5	11	NULL	0	NULL	statement 2	Process		is stronger than					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_20_8913_s_166	16199870	(A), delta50HA binds weakly (B), and delta26HA binds more strongly to the X chromosome than delta50HA (C); but staining intensity is consistently less than for MSL1NHA (Fig.  2C and D).	bind
10447	1	3369	7	11	NULL	0	NULL	delta50HA	GP		bind					 X chromosome 	Chromosome				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_20_8913_s_166	16199870	(A), delta50HA binds weakly (B), and delta26HA binds more strongly to the X chromosome than delta50HA (C); but staining intensity is consistently less than for MSL1NHA (Fig.  2C and D).	bind
10448	2	3369	7	11	NULL	0	NULL	delta26HA	GP		bind					X chromosome 	Chromosome				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_20_8913_s_166	16199870	(A), delta50HA binds weakly (B), and delta26HA binds more strongly to the X chromosome than delta50HA (C); but staining intensity is consistently less than for MSL1NHA (Fig.  2C and D).	bind
10449	3	3369	7	11	NULL	0	NULL	statement 1	Process		is weaker than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_20_8913_s_166	16199870	(A), delta50HA binds weakly (B), and delta26HA binds more strongly to the X chromosome than delta50HA (C); but staining intensity is consistently less than for MSL1NHA (Fig.  2C and D).	bind
80439	1	3369	11	NULL	NULL	0	NULL	delta50HA	Protein		binds to 		weakly			X chromosome	Chromosome				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_20_8913_s_166	16199870	(A), delta50HA binds weakly (B), and delta26HA binds more strongly to the X chromosome than delta50HA (C); but staining intensity is consistently less than for MSL1NHA (Fig.  2C and D).	bind
80440	2	3369	11	NULL	NULL	0	NULL	delta26HA	Protein		binds to 		strongly			X chromosome	Chromosome				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_20_8913_s_166	16199870	(A), delta50HA binds weakly (B), and delta26HA binds more strongly to the X chromosome than delta50HA (C); but staining intensity is consistently less than for MSL1NHA (Fig.  2C and D).	bind
8500	1	3370	5	11	NULL	0	NULL	myosin	GP		bind					UNC-45	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_295_5555_669_s_66	11809970	(A), except that  they were incubated at 30 degrees C for 30 min. Myosin bound both UNC-45 and  Hsp90.	bind
8501	2	3370	5	11	NULL	0	NULL	myosin	GP		bind					Hsp90	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_295_5555_669_s_66	11809970	(A), except that  they were incubated at 30 degrees C for 30 min. Myosin bound both UNC-45 and  Hsp90.	bind
10450	1	3370	7	11	NULL	0	NULL	Myosin	GP		bind					UNC-45 	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_295_5555_669_s_66	11809970	(A), except that  they were incubated at 30 degrees C for 30 min. Myosin bound both UNC-45 and  Hsp90.	bind
10451	2	3370	7	11	NULL	0	NULL	Myosin	GP		bind					Hsp90	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_295_5555_669_s_66	11809970	(A), except that  they were incubated at 30 degrees C for 30 min. Myosin bound both UNC-45 and  Hsp90.	bind
80442	1	3370	11	NULL	NULL	0	NULL	Myosin	Protein		binds to 					UNC-45	Protein				NULL		0	NULL	NULL	NULL	gw60_science_295_5555_669_s_66	11809970	(A), except that  they were incubated at 30 degrees C for 30 min. Myosin bound both UNC-45 and  Hsp90.	bind
80443	2	3370	11	NULL	NULL	0	NULL	Myosin	Protein		binds to 					Hsp90	Protein				NULL		0	NULL	NULL	NULL	gw60_science_295_5555_669_s_66	11809970	(A), except that  they were incubated at 30 degrees C for 30 min. Myosin bound both UNC-45 and  Hsp90.	bind
8502	1	3375	5	11	NULL	0	NULL	Ser	AminoAcid		bind					Tsr	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_48_17354_s_65	16293695	(A), in response to two stimuli, Ser and MeAsp, which bind to Tsr and Tar, respectively.	bind
8503	2	3375	5	11	NULL	0	NULL	MeAsp	AminoAcid		bind					Tar	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_48_17354_s_65	16293695	(A), in response to two stimuli, Ser and MeAsp, which bind to Tsr and Tar, respectively.	bind
10569	1	3375	7	11	NULL	0	NULL	Ser	AminoAcid		bind					Tsr	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_48_17354_s_65	16293695	(A), in response to two stimuli, Ser and MeAsp, which bind to Tsr and Tar, respectively.	bind
10570	2	3375	7	11	NULL	0	NULL	MeAsp	AminoAcid		bind					Tar	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_48_17354_s_65	16293695	(A), in response to two stimuli, Ser and MeAsp, which bind to Tsr and Tar, respectively.	bind
80453	1	3375	11	NULL	NULL	0	NULL	Ser	AminoAcid		binds to 					Tsr	Protein				NULL		0	NULL	NULL	NULL	gw70_pnas_102_48_17354_s_65	16293695	(A), in response to two stimuli, Ser and MeAsp, which bind to Tsr and Tar, respectively.	bind
80454	2	3375	11	NULL	NULL	0	NULL	MeAsp	AminoAcid		binds to 					Tar	Protein				NULL		0	NULL	NULL	NULL	gw70_pnas_102_48_17354_s_65	16293695	(A), in response to two stimuli, Ser and MeAsp, which bind to Tsr and Tar, respectively.	bind
8504	1	3376	5	11	NULL	0	NULL	KLC	GP		bind					KHC	GP				NULL	subcortical microtubule array nucleates particles	NULL	NULL	NULL	NULL	gw70_development_130_22_5425_s_301	14507779	(A), KLC bound to KHC on [[ the subcortical microtubule  array nucleates particles ]] that include GBP and its binding partner Dsh.	bind
8505	2	3376	5	11	NULL	0	NULL	GBP	GP		bind					Dsh	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_130_22_5425_s_301	14507779	(A), KLC bound to KHC on [[ the subcortical microtubule  array nucleates particles ]] that include GBP and its binding partner Dsh.	bind
8507	3	3376	5	11	NULL	0	NULL	statement 1	Process		include					GBP	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_130_22_5425_s_301	14507779	(A), KLC bound to KHC on [[ the subcortical microtubule  array nucleates particles ]] that include GBP and its binding partner Dsh.	bind
8508	4	3376	5	11	NULL	0	NULL	statement 1	Process		include					Dsh	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_130_22_5425_s_301	14507779	(A), KLC bound to KHC on [[ the subcortical microtubule  array nucleates particles ]] that include GBP and its binding partner Dsh.	bind
10572	1	3376	7	11	NULL	0	NULL	KLC	GP		bind					KHC	GP				NULL	subcortical microtubule array nucleates particles	NULL	NULL	NULL	NULL	gw70_development_130_22_5425_s_301	14507779	(A), KLC bound to KHC on [[ the subcortical microtubule  array nucleates particles ]] that include GBP and its binding partner Dsh.	bind
10574	2	3376	7	11	NULL	0	NULL	GBP	GP		bind					Dsh	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_130_22_5425_s_301	14507779	(A), KLC bound to KHC on [[ the subcortical microtubule  array nucleates particles ]] that include GBP and its binding partner Dsh.	bind
10575	3	3376	7	11	NULL	0	NULL	statement 1	Process		include					GBP	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_130_22_5425_s_301	14507779	(A), KLC bound to KHC on [[ the subcortical microtubule  array nucleates particles ]] that include GBP and its binding partner Dsh.	bind
10576	4	3376	7	11	NULL	0	NULL	statement 1	Process		include					Dsh	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_130_22_5425_s_301	14507779	(A), KLC bound to KHC on [[ the subcortical microtubule  array nucleates particles ]] that include GBP and its binding partner Dsh.	bind
80481	1	3376	11	NULL	NULL	0	NULL	KLC	PartOfProtein		binds to 					KHC	PartOfProtein				NULL	subcortical microtubule	0	NULL	NULL	NULL	gw70_development_130_22_5425_s_301	14507779	(A), KLC bound to KHC on [[ the subcortical microtubule  array nucleates particles ]] that include GBP and its binding partner Dsh.	bind
80482	2	3376	11	NULL	NULL	0	NULL	statement 1	Process		nucleates					GBP	Protein				NULL		0	NULL	NULL	NULL	gw70_development_130_22_5425_s_301	14507779	(A), KLC bound to KHC on [[ the subcortical microtubule  array nucleates particles ]] that include GBP and its binding partner Dsh.	bind
80483	3	3376	11	NULL	NULL	0	NULL	statement 1	Process		nucleates					GBP	Protein				NULL		0	NULL	NULL	NULL	gw70_development_130_22_5425_s_301	14507779	(A), KLC bound to KHC on [[ the subcortical microtubule  array nucleates particles ]] that include GBP and its binding partner Dsh.	bind
80484	4	3376	11	NULL	NULL	0	NULL	Dsh	Protein		is a binding partner of 					GBP	Protein				NULL		0	NULL	NULL	NULL	gw70_development_130_22_5425_s_301	14507779	(A), KLC bound to KHC on [[ the subcortical microtubule  array nucleates particles ]] that include GBP and its binding partner Dsh.	bind
8509	1	3378	5	11	NULL	0	NULL	SP-B21 cells	Cell	anti-CD3-stimulated	bind					IL-5	GP			RE-II	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_26_16453_s_256	9195954	(A), NF-Y(B), and c-Jun transcription factors were tested for the ability to recognize specific proteins from anti-CD3-stimulated SP-B21 cells bound to IL-5 RE-II in EMSAs.	bind
10578	1	3378	7	11	NULL	0	NULL	 SP-B21 cells	Cell	anti-CD3-stimulated	bind					IL-5 	GP			RE-II	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_26_16453_s_256	9195954	(A), NF-Y(B), and c-Jun transcription factors were tested for the ability to recognize specific proteins from anti-CD3-stimulated SP-B21 cells bound to IL-5 RE-II in EMSAs.	bind
80485	1	3378	11	NULL	NULL	0	NULL	NF-Y	Protein		is a type of 					transcription factor	Protein				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_26_16453_s_256	9195954	(A), NF-Y(B), and c-Jun transcription factors were tested for the ability to recognize specific proteins from anti-CD3-stimulated SP-B21 cells bound to IL-5 RE-II in EMSAs.	bind
80486	2	3378	11	NULL	NULL	0	NULL	c-Jun	Protein		is a type of 					transcription factor	Protein				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_26_16453_s_256	9195954	(A), NF-Y(B), and c-Jun transcription factors were tested for the ability to recognize specific proteins from anti-CD3-stimulated SP-B21 cells bound to IL-5 RE-II in EMSAs.	bind
80487	3	3378	11	NULL	NULL	0	NULL	anti-CD3	PartOfProtein		stimulates					SP-B21 cells	Cell				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_26_16453_s_256	9195954	(A), NF-Y(B), and c-Jun transcription factors were tested for the ability to recognize specific proteins from anti-CD3-stimulated SP-B21 cells bound to IL-5 RE-II in EMSAs.	bind
80488	4	3378	11	NULL	NULL	0	NULL	SP-B21 cell	cell		binds to 					IL-5 RE-II	PartOfProtein				NULL	in EMSAs	0	NULL	NULL	NULL	gw60_jbiolchem_272_26_16453_s_256	9195954	(A), NF-Y(B), and c-Jun transcription factors were tested for the ability to recognize specific proteins from anti-CD3-stimulated SP-B21 cells bound to IL-5 RE-II in EMSAs.	bind
10582	1	3381	7	11	NULL	0	NULL	P-selectin	GP		bind					fibrinogen	GP				NULL	 circulating platelets	NULL	NULL	NULL	NULL	gw60_circulation_93_2_229_s_112	8548893	(A), P-selectin (B), bound fibrinogen (C), and activated fibrinogen receptor (D) on circulating platelets in AMI patients (n=15) before and after (4, 8, 24, and 48 hours) successful recanalization of the infarct-related vessel ( ).	bind
10583	2	3381	7	11	NULL	0	NULL	statement 1	Process		activates					fibrinogen receptor	GP				NULL	circulating platelets	NULL	NULL	NULL	NULL	gw60_circulation_93_2_229_s_112	8548893	(A), P-selectin (B), bound fibrinogen (C), and activated fibrinogen receptor (D) on circulating platelets in AMI patients (n=15) before and after (4, 8, 24, and 48 hours) successful recanalization of the infarct-related vessel ( ).	bind
80489	1	3381	11	NULL	NULL	0	NULL	P-selectin	Protein		expressed on					circulating platelets	CellComponent				NULL	in AMI patients	0	NULL	NULL	NULL	gw60_circulation_93_2_229_s_112	8548893	(A), P-selectin (B), bound fibrinogen (C), and activated fibrinogen receptor (D) on circulating platelets in AMI patients (n=15) before and after (4, 8, 24, and 48 hours) successful recanalization of the infarct-related vessel ( ).	bind
80490	2	3381	11	NULL	NULL	0	NULL	fibrinogen	Protein	bound	expressed on					circulating platelets	CellComponent				NULL	in AMI patients	0	NULL	NULL	NULL	gw60_circulation_93_2_229_s_112	8548893	(A), P-selectin (B), bound fibrinogen (C), and activated fibrinogen receptor (D) on circulating platelets in AMI patients (n=15) before and after (4, 8, 24, and 48 hours) successful recanalization of the infarct-related vessel ( ).	bind
80491	3	3381	11	NULL	NULL	0	NULL	fibrinogen receptor	Protein	active	expressed on					circulating platelets	CellComponent				NULL	in AMI patients	0	NULL	NULL	NULL	gw60_circulation_93_2_229_s_112	8548893	(A), P-selectin (B), bound fibrinogen (C), and activated fibrinogen receptor (D) on circulating platelets in AMI patients (n=15) before and after (4, 8, 24, and 48 hours) successful recanalization of the infarct-related vessel ( ).	bind
8510	1	3385	5	11	NULL	0	NULL	Stx1	GP		bind					granulocyte cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_11_6680_s_79	15501802	(A), Stx1 (B), and Stx2 (C) binding to cells on granulocyte  smears are shown.	bind
8511	2	3385	5	11	NULL	0	NULL	Stx2	GP		bind					granulocyte cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_11_6680_s_79	15501802	(A), Stx1 (B), and Stx2 (C) binding to cells on granulocyte  smears are shown.	bind
10584	1	3385	7	11	NULL	0	NULL	Stx1	GP		binds					granulocyte cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_11_6680_s_79	15501802	(A), Stx1 (B), and Stx2 (C) binding to cells on granulocyte  smears are shown.	bind
10585	2	3385	7	11	NULL	0	NULL	Stx2	GP		bind					granulocyte cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_11_6680_s_79	15501802	(A), Stx1 (B), and Stx2 (C) binding to cells on granulocyte  smears are shown.	bind
80492	1	3385	11	NULL	NULL	0	NULL	 Stx1	Protein		binds to 					granulocyte	Cell				NULL		0	NULL	NULL	NULL	gw70_infectimmun_72_11_6680_s_79	15501802	(A), Stx1 (B), and Stx2 (C) binding to cells on granulocyte  smears are shown.	bind
80493	2	3385	11	NULL	NULL	0	NULL	Stx2	Protein		binds to 					granulocyte	Cell				NULL		0	NULL	NULL	NULL	gw70_infectimmun_72_11_6680_s_79	15501802	(A), Stx1 (B), and Stx2 (C) binding to cells on granulocyte  smears are shown.	bind
8512	1	3388	5	11	NULL	0	NULL	MMP-2	GP	active	bind			HP		endostatin	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_febslett_519_1_147_s_113	12023034	(A), the active MMP-2 HP (B), and the GST-fused MMP-2 HP domain (C) binding to the immobilized endostatin (thick line) or TIMP-2 as a control (thin line) were shown.	bind
8513	2	3388	5	11	NULL	0	NULL	MMP-2	GP	active	bind			HP		TIMP-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_519_1_147_s_113	12023034	(A), the active MMP-2 HP (B), and the GST-fused MMP-2 HP domain (C) binding to the immobilized endostatin (thick line) or TIMP-2 as a control (thin line) were shown.	bind
8514	3	3388	5	11	NULL	0	NULL	MMP-2	GP	GST-fused	bind			HP domain		endostatin	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_febslett_519_1_147_s_113	12023034	(A), the active MMP-2 HP (B), and the GST-fused MMP-2 HP domain (C) binding to the immobilized endostatin (thick line) or TIMP-2 as a control (thin line) were shown.	bind
8515	4	3388	5	11	NULL	0	NULL	MMP-2	GP	GST-fused	bind			HP domain		TIMP-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_519_1_147_s_113	12023034	(A), the active MMP-2 HP (B), and the GST-fused MMP-2 HP domain (C) binding to the immobilized endostatin (thick line) or TIMP-2 as a control (thin line) were shown.	bind
10586	1	3388	7	11	NULL	0	NULL	MMP-2 	GP	active	bind			HP		endostatin 	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_febslett_519_1_147_s_113	12023034	(A), the active MMP-2 HP (B), and the GST-fused MMP-2 HP domain (C) binding to the immobilized endostatin (thick line) or TIMP-2 as a control (thin line) were shown.	bind
10587	2	3388	7	11	NULL	0	NULL	MMP-2	GP	active	bind			HP		TIMP-2 	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_519_1_147_s_113	12023034	(A), the active MMP-2 HP (B), and the GST-fused MMP-2 HP domain (C) binding to the immobilized endostatin (thick line) or TIMP-2 as a control (thin line) were shown.	bind
10588	3	3388	7	11	NULL	0	NULL	MMP-2	GP	GST-fused 	bind			HP		endostatin 	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_febslett_519_1_147_s_113	12023034	(A), the active MMP-2 HP (B), and the GST-fused MMP-2 HP domain (C) binding to the immobilized endostatin (thick line) or TIMP-2 as a control (thin line) were shown.	bind
10589	4	3388	7	11	NULL	0	NULL	MMP-2	GP	GST-fused 	bind			HP		TIMP-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_519_1_147_s_113	12023034	(A), the active MMP-2 HP (B), and the GST-fused MMP-2 HP domain (C) binding to the immobilized endostatin (thick line) or TIMP-2 as a control (thin line) were shown.	bind
80494	1	3388	11	NULL	NULL	0	NULL	MMP-2 HP	Protein	active	binds to 					endostatin	Protein	immobilized			NULL		0	NULL	NULL	NULL	gw60_febslett_519_1_147_s_113	12023034	(A), the active MMP-2 HP (B), and the GST-fused MMP-2 HP domain (C) binding to the immobilized endostatin (thick line) or TIMP-2 as a control (thin line) were shown.	bind
80495	2	3388	11	NULL	NULL	0	NULL	GST	Protein		fused to					MMP-2 HP	Protein				NULL		0	NULL	NULL	NULL	gw60_febslett_519_1_147_s_113	12023034	(A), the active MMP-2 HP (B), and the GST-fused MMP-2 HP domain (C) binding to the immobilized endostatin (thick line) or TIMP-2 as a control (thin line) were shown.	bind
80496	3	3388	11	NULL	NULL	0	NULL	statement 2	Protein		binds to 					endostatin	Protein	immobilized			NULL		0	NULL	NULL	NULL	gw60_febslett_519_1_147_s_113	12023034	(A), the active MMP-2 HP (B), and the GST-fused MMP-2 HP domain (C) binding to the immobilized endostatin (thick line) or TIMP-2 as a control (thin line) were shown.	bind
80497	4	3388	11	NULL	NULL	0	NULL	MMP-2 HP	Protein	active	binds to 					TIMP-2	Protein				NULL		0	NULL	NULL	NULL	gw60_febslett_519_1_147_s_113	12023034	(A), the active MMP-2 HP (B), and the GST-fused MMP-2 HP domain (C) binding to the immobilized endostatin (thick line) or TIMP-2 as a control (thin line) were shown.	bind
80498	5	3388	11	NULL	NULL	0	NULL	statement 2	Protein		binds to 					TIMP-2	Protein				NULL		0	NULL	NULL	NULL	gw60_febslett_519_1_147_s_113	12023034	(A), the active MMP-2 HP (B), and the GST-fused MMP-2 HP domain (C) binding to the immobilized endostatin (thick line) or TIMP-2 as a control (thin line) were shown.	bind
80499	1	3389	11	NULL	NULL	0	NULL	TIM-1-578	Protein		binds to 					GST-PER	Protein	beads			NULL		0	NULL	NULL	NULL	gw60_neuron_17_5_911_s_175	8938123	(A), TIM-1-578 (B), TIM-715-1389 (C), TIM-914-1389 (D), and TIM-1-914 (E) that bound to the indicated GST-PER beads were detected by autoradiography.	bind
80500	2	3389	11	NULL	NULL	0	NULL	TIM-715-1389	Protein		binds to 					GST-PER	Protein	beads			NULL		0	NULL	NULL	NULL	gw60_neuron_17_5_911_s_175	8938123	(A), TIM-1-578 (B), TIM-715-1389 (C), TIM-914-1389 (D), and TIM-1-914 (E) that bound to the indicated GST-PER beads were detected by autoradiography.	bind
80501	3	3389	11	NULL	NULL	0	NULL	TIM-914-1389	Protein		binds to 					GST-PER	Protein	beads			NULL		0	NULL	NULL	NULL	gw60_neuron_17_5_911_s_175	8938123	(A), TIM-1-578 (B), TIM-715-1389 (C), TIM-914-1389 (D), and TIM-1-914 (E) that bound to the indicated GST-PER beads were detected by autoradiography.	bind
80502	4	3389	11	NULL	NULL	0	NULL	TIM-1-914	Protein		binds to 					GST-PER	Protein	beads			NULL		0	NULL	NULL	NULL	gw60_neuron_17_5_911_s_175	8938123	(A), TIM-1-578 (B), TIM-715-1389 (C), TIM-914-1389 (D), and TIM-1-914 (E) that bound to the indicated GST-PER beads were detected by autoradiography.	bind
80503	5	3389	11	NULL	NULL	0	NULL	statement 1	Process		detected by					autoradiography	ResearchActivity				NULL		0	NULL	NULL	NULL	gw60_neuron_17_5_911_s_175	8938123	(A), TIM-1-578 (B), TIM-715-1389 (C), TIM-914-1389 (D), and TIM-1-914 (E) that bound to the indicated GST-PER beads were detected by autoradiography.	bind
80504	6	3389	11	NULL	NULL	0	NULL	statement 2	Process		detected by					autoradiography	ResearchActivity				NULL		0	NULL	NULL	NULL	gw60_neuron_17_5_911_s_175	8938123	(A), TIM-1-578 (B), TIM-715-1389 (C), TIM-914-1389 (D), and TIM-1-914 (E) that bound to the indicated GST-PER beads were detected by autoradiography.	bind
80505	7	3389	11	NULL	NULL	0	NULL	statement 3	Process		detected by					autoradiography	ResearchActivity				NULL		0	NULL	NULL	NULL	gw60_neuron_17_5_911_s_175	8938123	(A), TIM-1-578 (B), TIM-715-1389 (C), TIM-914-1389 (D), and TIM-1-914 (E) that bound to the indicated GST-PER beads were detected by autoradiography.	bind
80506	8	3389	11	NULL	NULL	0	NULL	statement 4	Process		detected by					autoradiography	ResearchActivity				NULL		0	NULL	NULL	NULL	gw60_neuron_17_5_911_s_175	8938123	(A), TIM-1-578 (B), TIM-715-1389 (C), TIM-914-1389 (D), and TIM-1-914 (E) that bound to the indicated GST-PER beads were detected by autoradiography.	bind
8516	1	3390	5	11	NULL	0	NULL	VLA-4	GP		bind					VCAM-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_2_153_s_95	10904000	(A), treated with mAb Lia (nonblocking control) (B), mAb HP1/3 (anti-VLA-4, blocking FN binding) (C), vessel treated with mAb MK-2.7 to VCAM-1 (D), ILDV peptide present during perfusion (E), HP1/2 blocking VLA-4 binding to VCAM-1, and FN (F).	bind
8517	2	3390	5	11	NULL	0	NULL	VLA-4	GP		bind					FN	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_2_153_s_95	10904000	(A), treated with mAb Lia (nonblocking control) (B), mAb HP1/3 (anti-VLA-4, blocking FN binding) (C), vessel treated with mAb MK-2.7 to VCAM-1 (D), ILDV peptide present during perfusion (E), HP1/2 blocking VLA-4 binding to VCAM-1, and FN (F).	bind
8518	3	3390	5	11	NULL	0	NULL	HP1/2	GP		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_2_153_s_95	10904000	(A), treated with mAb Lia (nonblocking control) (B), mAb HP1/3 (anti-VLA-4, blocking FN binding) (C), vessel treated with mAb MK-2.7 to VCAM-1 (D), ILDV peptide present during perfusion (E), HP1/2 blocking VLA-4 binding to VCAM-1, and FN (F).	bind
8519	4	3390	5	11	NULL	0	NULL	HP1/2	GP		blocks					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_2_153_s_95	10904000	(A), treated with mAb Lia (nonblocking control) (B), mAb HP1/3 (anti-VLA-4, blocking FN binding) (C), vessel treated with mAb MK-2.7 to VCAM-1 (D), ILDV peptide present during perfusion (E), HP1/2 blocking VLA-4 binding to VCAM-1, and FN (F).	bind
10593	1	3390	7	11	NULL	0	NULL	VLA-4	GP		bind					VCAM-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_2_153_s_95	10904000	(A), treated with mAb Lia (nonblocking control) (B), mAb HP1/3 (anti-VLA-4, blocking FN binding) (C), vessel treated with mAb MK-2.7 to VCAM-1 (D), ILDV peptide present during perfusion (E), HP1/2 blocking VLA-4 binding to VCAM-1, and FN (F).	bind
10594	2	3390	7	11	NULL	0	NULL	VLA-4	GP		bind					FN	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_2_153_s_95	10904000	(A), treated with mAb Lia (nonblocking control) (B), mAb HP1/3 (anti-VLA-4, blocking FN binding) (C), vessel treated with mAb MK-2.7 to VCAM-1 (D), ILDV peptide present during perfusion (E), HP1/2 blocking VLA-4 binding to VCAM-1, and FN (F).	bind
14951	3	3390	7	11	NULL	0	NULL	HP1/2	GP		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_2_153_s_95	10904000	(A), treated with mAb Lia (nonblocking control) (B), mAb HP1/3 (anti-VLA-4, blocking FN binding) (C), vessel treated with mAb MK-2.7 to VCAM-1 (D), ILDV peptide present during perfusion (E), HP1/2 blocking VLA-4 binding to VCAM-1, and FN (F).	bind
14952	4	3390	7	11	NULL	0	NULL	HP1/2	GP		blocks					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_2_153_s_95	10904000	(A), treated with mAb Lia (nonblocking control) (B), mAb HP1/3 (anti-VLA-4, blocking FN binding) (C), vessel treated with mAb MK-2.7 to VCAM-1 (D), ILDV peptide present during perfusion (E), HP1/2 blocking VLA-4 binding to VCAM-1, and FN (F).	bind
80507	1	3390	11	NULL	NULL	0	NULL	VLA-4	Protein		binds to 					VCAM-1	Protein				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_2_153_s_95	10904000	(A), treated with mAb Lia (nonblocking control) (B), mAb HP1/3 (anti-VLA-4, blocking FN binding) (C), vessel treated with mAb MK-2.7 to VCAM-1 (D), ILDV peptide present during perfusion (E), HP1/2 blocking VLA-4 binding to VCAM-1, and FN (F).	bind
80508	2	3390	11	NULL	NULL	0	NULL	VLA-4	Protein		binds to 					FN	Protein				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_2_153_s_95	10904000	(A), treated with mAb Lia (nonblocking control) (B), mAb HP1/3 (anti-VLA-4, blocking FN binding) (C), vessel treated with mAb MK-2.7 to VCAM-1 (D), ILDV peptide present during perfusion (E), HP1/2 blocking VLA-4 binding to VCAM-1, and FN (F).	bind
80509	3	3390	11	NULL	NULL	0	NULL	HP1/2	PartOfProtein		blocks					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_2_153_s_95	10904000	(A), treated with mAb Lia (nonblocking control) (B), mAb HP1/3 (anti-VLA-4, blocking FN binding) (C), vessel treated with mAb MK-2.7 to VCAM-1 (D), ILDV peptide present during perfusion (E), HP1/2 blocking VLA-4 binding to VCAM-1, and FN (F).	bind
80510	4	3390	11	NULL	NULL	0	NULL	HP1/2	PartOfProtein		blocks					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_2_153_s_95	10904000	(A), treated with mAb Lia (nonblocking control) (B), mAb HP1/3 (anti-VLA-4, blocking FN binding) (C), vessel treated with mAb MK-2.7 to VCAM-1 (D), ILDV peptide present during perfusion (E), HP1/2 blocking VLA-4 binding to VCAM-1, and FN (F).	bind
8520	1	3392	5	11	NULL	0	NULL	NXT1	GP		bind		preferentially			GTP-Ran	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8616_s_166	10567585	(A), whereas NXT1 preferentially bound GTP-Ran (B).	bind
10596	1	3392	7	11	NULL	0	NULL	NXT1	GP		bind		preferentially			GTP-Ran	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8616_s_166	10567585	(A), whereas NXT1 preferentially bound GTP-Ran (B).	bind
80511	1	3392	11	NULL	NULL	0	NULL	NXT1	Protein		binds to 					GTP-Ran	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_12_8616_s_166	10567585	(A), whereas NXT1 preferentially bound GTP-Ran (B).	bind
8521	1	3393	5	11	NULL	0	NULL	stem-loop IIIa	NucleicAcid		bind					GAPDH	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_24_14134_s_163	8662893	(A), whereas poly(C) had no apparent effect on stem-loop IIIa binding to GAPDH or p39.	bind
8522	2	3393	5	11	NULL	0	NULL	stem-loop IIIa	NucleicAcid		bind					p39	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_24_14134_s_163	8662893	(A), whereas poly(C) had no apparent effect on stem-loop IIIa binding to GAPDH or p39.	bind
8523	3	3393	5	11	NULL	0	NULL	poly(C)	NucleicAcid		does not effect					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_24_14134_s_163	8662893	(A), whereas poly(C) had no apparent effect on stem-loop IIIa binding to GAPDH or p39.	bind
8524	4	3393	5	11	NULL	0	NULL	poly(C)	NucleicAcid		does not effect					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_24_14134_s_163	8662893	(A), whereas poly(C) had no apparent effect on stem-loop IIIa binding to GAPDH or p39.	bind
8525	5	3393	5	11	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_24_14134_s_163	8662893	(A), whereas poly(C) had no apparent effect on stem-loop IIIa binding to GAPDH or p39.	bind
10597	1	3393	7	11	NULL	0	NULL	stem-loop IIIa	NucleicAcid		bind					GAPDH	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_24_14134_s_163	8662893	(A), whereas poly(C) had no apparent effect on stem-loop IIIa binding to GAPDH or p39.	bind
10598	2	3393	7	11	NULL	0	NULL	stem-loop IIIa	NucleicAcid		bind					p39	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_24_14134_s_163	8662893	(A), whereas poly(C) had no apparent effect on stem-loop IIIa binding to GAPDH or p39.	bind
10599	3	3393	7	11	NULL	0	NULL	poly(C)	NucleicAcid		does not effect					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_24_14134_s_163	8662893	(A), whereas poly(C) had no apparent effect on stem-loop IIIa binding to GAPDH or p39.	bind
10600	4	3393	7	11	NULL	0	NULL	poly(C)	NucleicAcid		does not effect					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_24_14134_s_163	8662893	(A), whereas poly(C) had no apparent effect on stem-loop IIIa binding to GAPDH or p39.	bind
80512	1	3393	11	NULL	NULL	0	NULL	stem-loop IIIa	NucleicAcidSubstance		binds to 					GAPDH	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_24_14134_s_163	8662893	(A), whereas poly(C) had no apparent effect on stem-loop IIIa binding to GAPDH or p39.	bind
80513	2	3393	11	NULL	NULL	0	NULL	stem-loop IIIa	NucleicAcidSubstance		binds to 					p39	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_24_14134_s_163	8662893	(A), whereas poly(C) had no apparent effect on stem-loop IIIa binding to GAPDH or p39.	bind
8526	1	3396	5	11	NULL	0	NULL	Rab5	GP		bind					GST-GDI	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_2_421_s_55	11239470	(A), with 0-1  M GST-GDI and with or without 100  M ATP S. Rab5 bound to GST-GDI is compared to Rab5 remaining on endosomes after the experiment.	bind
10601	1	3396	7	11	NULL	0	NULL	Rab5	GP		bind					GST-GDI	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_2_421_s_55	11239470	(A), with 0-1  M GST-GDI and with or without 100  M ATP S. Rab5 bound to GST-GDI is compared to Rab5 remaining on endosomes after the experiment.	bind
80514	1	3396	11	NULL	NULL	0	NULL	Rab5	Protein		binds to 					GST-GDI	Protein				NULL		0	NULL	NULL	NULL	gw60_molcell_7_2_421_s_55	11239470	(A), with 0-1  M GST-GDI and with or without 100  M ATP S. Rab5 bound to GST-GDI is compared to Rab5 remaining on endosomes after the experiment.	bind
80515	2	3396	11	NULL	NULL	0	NULL	Rab5	Protein		remaining on					endosomes	CellComponent				NULL		0	NULL	NULL	NULL	gw60_molcell_7_2_421_s_55	11239470	(A), with 0-1  M GST-GDI and with or without 100  M ATP S. Rab5 bound to GST-GDI is compared to Rab5 remaining on endosomes after the experiment.	bind
80516	1	3397	11	NULL	NULL	0	NULL	Pab1p	Protein		binds to 					eIF4G1	Protein		115 amino acid		NULL		0	NULL	NULL	NULL	gw60_embo_18_11_3153_s_277	10357826	(A), with 115 amino acid Pab1p-binding fragments of either eIF4G1 or eIF4G2 fused at their N-termini to glutathione  S-transferase (GST) (Tarun and Sachs, 1996  ; Tarun  et al., 1997  ).	bind
80517	2	3397	11	NULL	NULL	0	NULL	Pab1p	Protein		binds to 					eIF4G2	Protein		115 amino acid		NULL		0	NULL	NULL	NULL	gw60_embo_18_11_3153_s_277	10357826	(A), with 115 amino acid Pab1p-binding fragments of either eIF4G1 or eIF4G2 fused at their N-termini to glutathione  S-transferase (GST) (Tarun and Sachs, 1996  ; Tarun  et al., 1997  ).	bind
80518	3	3397	11	NULL	NULL	0	NULL	eIF4G1	Protein		fused to					glutathione S-transferase	Protein		N-termini		NULL		0	NULL	NULL	NULL	gw60_embo_18_11_3153_s_277	10357826	(A), with 115 amino acid Pab1p-binding fragments of either eIF4G1 or eIF4G2 fused at their N-termini to glutathione  S-transferase (GST) (Tarun and Sachs, 1996  ; Tarun  et al., 1997  ).	bind
80519	4	3397	11	NULL	NULL	0	NULL	eIF4G2	Protein		fused to					glutathione S-transferase	Protein		N-termini		NULL		0	NULL	NULL	NULL	gw60_embo_18_11_3153_s_277	10357826	(A), with 115 amino acid Pab1p-binding fragments of either eIF4G1 or eIF4G2 fused at their N-termini to glutathione  S-transferase (GST) (Tarun and Sachs, 1996  ; Tarun  et al., 1997  ).	bind
80520	5	3397	11	NULL	NULL	0	NULL	glutathione S-transferase	Protein		is					GST	Protein				NULL		0	NULL	NULL	NULL	gw60_embo_18_11_3153_s_277	10357826	(A), with 115 amino acid Pab1p-binding fragments of either eIF4G1 or eIF4G2 fused at their N-termini to glutathione  S-transferase (GST) (Tarun and Sachs, 1996  ; Tarun  et al., 1997  ).	bind
80521	1	3399	11	NULL	NULL	0	NULL	PABP	Protein		binds to 					 3' poly	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_annurevphytopathol_43_0_39_s_161	16078876	(A)-binding  protein (PABP) bound to the 3' poly	bind
7533	1	3401	6	11	NULL	0	NULL	hnRNPA1	GP		bind					single-stranded RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_17_14338_s_204	11278842	(A)-binding protein ( 19); and hnRNPA1 ( 16), which binds single-stranded RNA and the structure of the first two RBD of nucleolin bound to the NRE motif ( 20).	bind
7534	2	3401	6	11	NULL	0	NULL	nucleolin	GP		bind			RBD					NRE motif		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_17_14338_s_204	11278842	(A)-binding protein ( 19); and hnRNPA1 ( 16), which binds single-stranded RNA and the structure of the first two RBD of nucleolin bound to the NRE motif ( 20).	bind
10602	1	3401	7	11	NULL	0	NULL	hnRNPA1	GP		bind					single-stranded RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_17_14338_s_204	11278842	(A)-binding protein ( 19); and hnRNPA1 ( 16), which binds single-stranded RNA and the structure of the first two RBD of nucleolin bound to the NRE motif ( 20).	bind
10603	2	3401	7	11	NULL	0	NULL	 nucleolin	GP		bind			RBD					NRE motif		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_17_14338_s_204	11278842	(A)-binding protein ( 19); and hnRNPA1 ( 16), which binds single-stranded RNA and the structure of the first two RBD of nucleolin bound to the NRE motif ( 20).	bind
80522	1	3401	11	NULL	NULL	0	NULL	hnRNPA1	Protein		binds to 					RNA	NucleicAcidSubstance	single-stranded			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_17_14338_s_204	11278842	(A)-binding protein ( 19); and hnRNPA1 ( 16), which binds single-stranded RNA and the structure of the first two RBD of nucleolin bound to the NRE motif ( 20).	bind
80523	2	3401	11	NULL	NULL	0	NULL	nucleolin	Protein		binds to 			RBD					NRE motif		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_17_14338_s_204	11278842	(A)-binding protein ( 19); and hnRNPA1 ( 16), which binds single-stranded RNA and the structure of the first two RBD of nucleolin bound to the NRE motif ( 20).	bind
7536	1	3402	6	11	NULL	0	NULL	nucleolin	GP		bind								RRM		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4765_s_221	10848602	(A)-binding protein ( 7), nucleolin ( 50), SF2 (also known as ASF) ( 8), and U2AF ( 56), binding by a single RRM is much weaker and/or less specific than binding by a combination of two or more RRMs.	bind
7537	2	3402	6	11	NULL	0	NULL	SF2	GP		bind								RRM		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4765_s_221	10848602	(A)-binding protein ( 7), nucleolin ( 50), SF2 (also known as ASF) ( 8), and U2AF ( 56), binding by a single RRM is much weaker and/or less specific than binding by a combination of two or more RRMs.	bind
7538	3	3402	6	11	NULL	0	NULL	SF2	GP		is					ASF	GP	a synonym of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4765_s_221	10848602	(A)-binding protein ( 7), nucleolin ( 50), SF2 (also known as ASF) ( 8), and U2AF ( 56), binding by a single RRM is much weaker and/or less specific than binding by a combination of two or more RRMs.	bind
7539	4	3402	6	11	NULL	0	NULL	U2AF	GP		bind								RRM		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4765_s_221	10848602	(A)-binding protein ( 7), nucleolin ( 50), SF2 (also known as ASF) ( 8), and U2AF ( 56), binding by a single RRM is much weaker and/or less specific than binding by a combination of two or more RRMs.	bind
10604	1	3402	7	11	NULL	0	NULL	nucleolin	GP		bind								RRM		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4765_s_221	10848602	(A)-binding protein ( 7), nucleolin ( 50), SF2 (also known as ASF) ( 8), and U2AF ( 56), binding by a single RRM is much weaker and/or less specific than binding by a combination of two or more RRMs.	bind
10605	2	3402	7	11	NULL	0	NULL	SF2	GP		bind								RRM		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4765_s_221	10848602	(A)-binding protein ( 7), nucleolin ( 50), SF2 (also known as ASF) ( 8), and U2AF ( 56), binding by a single RRM is much weaker and/or less specific than binding by a combination of two or more RRMs.	bind
10606	3	3402	7	11	NULL	0	NULL	U2AF	GP		bind								RRM		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4765_s_221	10848602	(A)-binding protein ( 7), nucleolin ( 50), SF2 (also known as ASF) ( 8), and U2AF ( 56), binding by a single RRM is much weaker and/or less specific than binding by a combination of two or more RRMs.	bind
10608	4	3402	7	11	NULL	0	NULL	SF2	GP		is					ASF	GP	a synonym of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4765_s_221	10848602	(A)-binding protein ( 7), nucleolin ( 50), SF2 (also known as ASF) ( 8), and U2AF ( 56), binding by a single RRM is much weaker and/or less specific than binding by a combination of two or more RRMs.	bind
80524	1	3402	11	NULL	NULL	0	NULL	SF2	Protein		is					ASF	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_13_4765_s_221	10848602	(A)-binding protein ( 7), nucleolin ( 50), SF2 (also known as ASF) ( 8), and U2AF ( 56), binding by a single RRM is much weaker and/or less specific than binding by a combination of two or more RRMs.	bind
80525	2	3402	11	NULL	NULL	0	NULL	nucleolin	Protein		binds to 		weakly;;less specific						single RRM		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_13_4765_s_221	10848602	(A)-binding protein ( 7), nucleolin ( 50), SF2 (also known as ASF) ( 8), and U2AF ( 56), binding by a single RRM is much weaker and/or less specific than binding by a combination of two or more RRMs.	bind
80526	3	3402	11	NULL	NULL	0	NULL	SF2	Protein		binds to 		weakly;;less specific						single RRM		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_13_4765_s_221	10848602	(A)-binding protein ( 7), nucleolin ( 50), SF2 (also known as ASF) ( 8), and U2AF ( 56), binding by a single RRM is much weaker and/or less specific than binding by a combination of two or more RRMs.	bind
80527	4	3402	11	NULL	NULL	0	NULL	U2AF	Protein		binds to 		weakly;;less specific						single RRM		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_13_4765_s_221	10848602	(A)-binding protein ( 7), nucleolin ( 50), SF2 (also known as ASF) ( 8), and U2AF ( 56), binding by a single RRM is much weaker and/or less specific than binding by a combination of two or more RRMs.	bind
7541	2	3404	6	11	NULL	0	NULL	PABP	GP		bind					eIF4A	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_7_4449_s_20	12475969	(A)-binding protein (PABP) and a C-terminal fragment (cpC) that binds eIF4A and eIF3 ( ) (see Fig.  1).	bind
7542	3	3404	6	11	NULL	0	NULL	PABP	GP		bind					eIF3	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_7_4449_s_20	12475969	(A)-binding protein (PABP) and a C-terminal fragment (cpC) that binds eIF4A and eIF3 ( ) (see Fig.  1).	bind
7543	4	3404	6	11	NULL	0	NULL	cpC	AminoAcid		is					C-terminal fragment	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_7_4449_s_20	12475969	(A)-binding protein (PABP) and a C-terminal fragment (cpC) that binds eIF4A and eIF3 ( ) (see Fig.  1).	bind
7544	5	3404	6	11	NULL	0	NULL				bind			cpC		eIF4A	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_7_4449_s_20	12475969	(A)-binding protein (PABP) and a C-terminal fragment (cpC) that binds eIF4A and eIF3 ( ) (see Fig.  1).	bind
7545	6	3404	6	11	NULL	0	NULL				bind			cpC		eIF3	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_7_4449_s_20	12475969	(A)-binding protein (PABP) and a C-terminal fragment (cpC) that binds eIF4A and eIF3 ( ) (see Fig.  1).	bind
10609	1	3404	7	11	NULL	0	NULL	PABP	GP		bind					 eIF4A	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_7_4449_s_20	12475969	(A)-binding protein (PABP) and a C-terminal fragment (cpC) that binds eIF4A and eIF3 ( ) (see Fig.  1).	bind
10610	2	3404	7	11	NULL	0	NULL	PABP	GP		bind					eIF3	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_7_4449_s_20	12475969	(A)-binding protein (PABP) and a C-terminal fragment (cpC) that binds eIF4A and eIF3 ( ) (see Fig.  1).	bind
10611	3	3404	7	11	NULL	0	NULL				bind			C-terminal fragment		eIF4A	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_7_4449_s_20	12475969	(A)-binding protein (PABP) and a C-terminal fragment (cpC) that binds eIF4A and eIF3 ( ) (see Fig.  1).	bind
10612	4	3404	7	11	NULL	0	NULL				bind			C-terminal fragment		eIF3	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_7_4449_s_20	12475969	(A)-binding protein (PABP) and a C-terminal fragment (cpC) that binds eIF4A and eIF3 ( ) (see Fig.  1).	bind
10613	5	3404	7	11	NULL	0	NULL	C-terminal fragment	AminoAcid		is					cpC	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_7_4449_s_20	12475969	(A)-binding protein (PABP) and a C-terminal fragment (cpC) that binds eIF4A and eIF3 ( ) (see Fig.  1).	bind
80528	1	3404	11	NULL	NULL	0	NULL	PABP	Protein		binds to 					eIF4A	Protein				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_7_4449_s_20	12475969	(A)-binding protein (PABP) and a C-terminal fragment (cpC) that binds eIF4A and eIF3 ( ) (see Fig.  1).	bind
80529	2	3404	11	NULL	NULL	0	NULL	PABP	Protein		binds to 					eIF3	Protein				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_7_4449_s_20	12475969	(A)-binding protein (PABP) and a C-terminal fragment (cpC) that binds eIF4A and eIF3 ( ) (see Fig.  1).	bind
80530	3	3404	11	NULL	NULL	0	NULL				binds to 			C-terminal fragment		eIF4A	Protein				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_7_4449_s_20	12475969	(A)-binding protein (PABP) and a C-terminal fragment (cpC) that binds eIF4A and eIF3 ( ) (see Fig.  1).	bind
80531	4	3404	11	NULL	NULL	0	NULL				binds to 			C-terminal fragment		eIF3	Protein				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_7_4449_s_20	12475969	(A)-binding protein (PABP) and a C-terminal fragment (cpC) that binds eIF4A and eIF3 ( ) (see Fig.  1).	bind
80532	5	3404	11	NULL	NULL	0	NULL	C-terminal fragment	PartOfProtein		is					cpC	PartOfProtein				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_7_4449_s_20	12475969	(A)-binding protein (PABP) and a C-terminal fragment (cpC) that binds eIF4A and eIF3 ( ) (see Fig.  1).	bind
7547	1	3407	6	11	NULL	0	NULL	PABP	GP		bind					mRNA	NucleicAcid			ARS in 5''-untranslated region	NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_nucleic-acids-res_33_22_16356927_s_4	16356927	(A)-binding protein (PABP) mRNA translation involves  the binding of PABP to the adenine-rich autoregulatory sequence (ARS)  in the 5''-untranslated region of its own mRNA.	bind
7548	2	3407	6	11	NULL	0	NULL	ARS	NucleicAcid		is					adenine-rich autoregulatory sequence	NucleicAcid				NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_nucleic-acids-res_33_22_16356927_s_4	16356927	(A)-binding protein (PABP) mRNA translation involves  the binding of PABP to the adenine-rich autoregulatory sequence (ARS)  in the 5''-untranslated region of its own mRNA.	bind
7549	3	3407	6	11	NULL	0	NULL	PABP mRNA	NucleicAcid	translation of	involves					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_nucleic-acids-res_33_22_16356927_s_4	16356927	(A)-binding protein (PABP) mRNA translation involves  the binding of PABP to the adenine-rich autoregulatory sequence (ARS)  in the 5''-untranslated region of its own mRNA.	bind
10614	1	3407	7	11	NULL	0	NULL	PABP	GP		bind					mRNA	NucleicAcid			ARS in 5''-untranslated region	NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_nucleic-acids-res_33_22_16356927_s_4	16356927	(A)-binding protein (PABP) mRNA translation involves  the binding of PABP to the adenine-rich autoregulatory sequence (ARS)  in the 5''-untranslated region of its own mRNA.	bind
10615	2	3407	7	11	NULL	0	NULL	 adenine-rich autoregulatory sequence	NucleicAcid		is					ARS	NucleicAcid				NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_nucleic-acids-res_33_22_16356927_s_4	16356927	(A)-binding protein (PABP) mRNA translation involves  the binding of PABP to the adenine-rich autoregulatory sequence (ARS)  in the 5''-untranslated region of its own mRNA.	bind
52799	3	3407	7	11	NULL	0	NULL	PABP mRNA	NucleicAcid	translation of	involves					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_nucleic-acids-res_33_22_16356927_s_4	16356927	(A)-binding protein (PABP) mRNA translation involves  the binding of PABP to the adenine-rich autoregulatory sequence (ARS)  in the 5''-untranslated region of its own mRNA.	bind
80533	1	3407	11	NULL	NULL	0	NULL	PABP 	Protein		binds to 					PABP mRNA	NucleicAcidSubstance	adenine-rich autoregulatory sequence		5''-untranslated region	NULL		0	NULL	NULL	NULL	abs-batch0550-0559_nucleic-acids-res_33_22_16356927_s_4	16356927	(A)-binding protein (PABP) mRNA translation involves  the binding of PABP to the adenine-rich autoregulatory sequence (ARS)  in the 5''-untranslated region of its own mRNA.	bind
80534	2	3407	11	NULL	NULL	0	NULL	statement 1	Process		leads to					translation	MolecularProcess	PABP mRNA			NULL		0	NULL	NULL	NULL	abs-batch0550-0559_nucleic-acids-res_33_22_16356927_s_4	16356927	(A)-binding protein (PABP) mRNA translation involves  the binding of PABP to the adenine-rich autoregulatory sequence (ARS)  in the 5''-untranslated region of its own mRNA.	bind
7550	1	3409	6	11	NULL	0	NULL	p17M1234	NucleicAcid		is a type of					mutated RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2307_s_25	8999938	(A)-binding protein (PABP1) binds specifically to INS-1 within the p17 gag mRNA, but not to mutated RNA (p17M1234).	bind
7551	2	3409	6	11	NULL	0	NULL	PABP1	GP		bind		specifically			p17 gag mRNA	NucleicAcid			INS-1	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2307_s_25	8999938	(A)-binding protein (PABP1) binds specifically to INS-1 within the p17 gag mRNA, but not to mutated RNA (p17M1234).	bind
7552	3	3409	6	11	NULL	0	NULL	PABP1	GP		does not bind					p17M1234	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2307_s_25	8999938	(A)-binding protein (PABP1) binds specifically to INS-1 within the p17 gag mRNA, but not to mutated RNA (p17M1234).	bind
10616	1	3409	7	11	NULL	0	NULL	PABP1	GP		bind		specifically			p17 gag mRNA	NucleicAcid			INS-1	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2307_s_25	8999938	(A)-binding protein (PABP1) binds specifically to INS-1 within the p17 gag mRNA, but not to mutated RNA (p17M1234).	bind
10617	2	3409	7	11	NULL	0	NULL	PABP1	GP		does not bind					p17M1234	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2307_s_25	8999938	(A)-binding protein (PABP1) binds specifically to INS-1 within the p17 gag mRNA, but not to mutated RNA (p17M1234).	bind
10618	3	3409	7	11	NULL	0	NULL	p17M1234	NucleicAcid		is a type of					mutated RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2307_s_25	8999938	(A)-binding protein (PABP1) binds specifically to INS-1 within the p17 gag mRNA, but not to mutated RNA (p17M1234).	bind
80535	1	3409	11	NULL	NULL	NULL	NULL	PABP1	Protein		binds to 		specifically			statement 2	NucleicAcidSubstance				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2307_s_25	8999938	(A)-binding protein (PABP1) binds specifically to INS-1 within the p17 gag mRNA, but not to mutated RNA (p17M1234).	bind
80536	2	3409	11	NULL	NULL	0	NULL	INS-1	NucleicAcidSubstance		is within					p17 gag mRNA	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_4_2307_s_25	8999938	(A)-binding protein (PABP1) binds specifically to INS-1 within the p17 gag mRNA, but not to mutated RNA (p17M1234).	bind
80537	3	3409	11	NULL	NULL	0	NULL	PABP1	Protein		does not bind to					p17 gag mRNA	NucleicAcidSubstance	mutated		p17M1234	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_4_2307_s_25	8999938	(A)-binding protein (PABP1) binds specifically to INS-1 within the p17 gag mRNA, but not to mutated RNA (p17M1234).	bind
7554	2	3410	6	11	NULL	0	NULL	PABP1	GP		bind		preferentially			p17 gag mRNA	NucleicAcid			INS-1	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2307_s_6	8999938	(A)-binding protein 1 (PABP1) binds preferentially to INS-1 within the p17 gag mRNA, but not to a mutated mRNA in which INS-1 function is eliminated.	bind
7555	3	3410	6	11	NULL	0	NULL	p17 gag mRNA	NucleicAcid	mutant	lacks									INS-1	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2307_s_6	8999938	(A)-binding protein 1 (PABP1) binds preferentially to INS-1 within the p17 gag mRNA, but not to a mutated mRNA in which INS-1 function is eliminated.	bind
7556	4	3410	6	11	NULL	0	NULL	PABP1	GP		does not bind					statement 3	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2307_s_6	8999938	(A)-binding protein 1 (PABP1) binds preferentially to INS-1 within the p17 gag mRNA, but not to a mutated mRNA in which INS-1 function is eliminated.	bind
10619	1	3410	7	11	NULL	0	NULL	PABP1	GP		bind		preferentially			p17 gag mRNA	NucleicAcid			INS-1	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2307_s_6	8999938	(A)-binding protein 1 (PABP1) binds preferentially to INS-1 within the p17 gag mRNA, but not to a mutated mRNA in which INS-1 function is eliminated.	bind
10620	2	3410	7	11	NULL	0	NULL	PABP1	GP		does not bind					statement 3	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2307_s_6	8999938	(A)-binding protein 1 (PABP1) binds preferentially to INS-1 within the p17 gag mRNA, but not to a mutated mRNA in which INS-1 function is eliminated.	bind
10621	3	3410	7	11	NULL	0	NULL	p17 gag mRNA	NucleicAcid	mutant	lacks									INS-1	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2307_s_6	8999938	(A)-binding protein 1 (PABP1) binds preferentially to INS-1 within the p17 gag mRNA, but not to a mutated mRNA in which INS-1 function is eliminated.	bind
7557	1	3411	6	11	NULL	0	NULL	poly(U)-binding protein 1	GP		is					Pub1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_7752_s_48	11779864	(A)-binding protein 1), Pub1p (poly(U)-binding protein 1), Npl3p (nuclear protein localization 3), Hrp1p (hnRNP-like protein 1), and Nab2p (nuclear polyadenylated RNA binding 2), were identified in a screen for proteins that cross-link to polyadenylated RNA  in vivo ( 26,  27).	bind
7558	2	3411	6	11	NULL	0	NULL	Pub1p	GP		cross link to					RNA	NucleicAcid	polyadenylated			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_7752_s_48	11779864	(A)-binding protein 1), Pub1p (poly(U)-binding protein 1), Npl3p (nuclear protein localization 3), Hrp1p (hnRNP-like protein 1), and Nab2p (nuclear polyadenylated RNA binding 2), were identified in a screen for proteins that cross-link to polyadenylated RNA  in vivo ( 26,  27).	bind
7559	3	3411	6	11	NULL	0	NULL	Npl3p	GP		cross link to					RNA	NucleicAcid	polyadenylated			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_7752_s_48	11779864	(A)-binding protein 1), Pub1p (poly(U)-binding protein 1), Npl3p (nuclear protein localization 3), Hrp1p (hnRNP-like protein 1), and Nab2p (nuclear polyadenylated RNA binding 2), were identified in a screen for proteins that cross-link to polyadenylated RNA  in vivo ( 26,  27).	bind
7560	4	3411	6	11	NULL	0	NULL	hnRNP-like protein 1	GP		is					Hrp1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_7752_s_48	11779864	(A)-binding protein 1), Pub1p (poly(U)-binding protein 1), Npl3p (nuclear protein localization 3), Hrp1p (hnRNP-like protein 1), and Nab2p (nuclear polyadenylated RNA binding 2), were identified in a screen for proteins that cross-link to polyadenylated RNA  in vivo ( 26,  27).	bind
7561	5	3411	6	11	NULL	0	NULL	Hrp1p	GP		cross link to					RNA	NucleicAcid	polyadenylated			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_7752_s_48	11779864	(A)-binding protein 1), Pub1p (poly(U)-binding protein 1), Npl3p (nuclear protein localization 3), Hrp1p (hnRNP-like protein 1), and Nab2p (nuclear polyadenylated RNA binding 2), were identified in a screen for proteins that cross-link to polyadenylated RNA  in vivo ( 26,  27).	bind
7562	6	3411	6	11	NULL	0	NULL	nuclear polyadenylated RNA binding 2	GP		is					Nab2p	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_7752_s_48	11779864	(A)-binding protein 1), Pub1p (poly(U)-binding protein 1), Npl3p (nuclear protein localization 3), Hrp1p (hnRNP-like protein 1), and Nab2p (nuclear polyadenylated RNA binding 2), were identified in a screen for proteins that cross-link to polyadenylated RNA  in vivo ( 26,  27).	bind
7563	7	3411	6	11	NULL	0	NULL	Nab2p	GP		cross link to					RNA	NucleicAcid	polyadenylated			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_7752_s_48	11779864	(A)-binding protein 1), Pub1p (poly(U)-binding protein 1), Npl3p (nuclear protein localization 3), Hrp1p (hnRNP-like protein 1), and Nab2p (nuclear polyadenylated RNA binding 2), were identified in a screen for proteins that cross-link to polyadenylated RNA  in vivo ( 26,  27).	bind
52811	8	3411	6	11	NULL	0	NULL	Npl3p	GP		is					nuclear protein localization 3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_7752_s_48	11779864	(A)-binding protein 1), Pub1p (poly(U)-binding protein 1), Npl3p (nuclear protein localization 3), Hrp1p (hnRNP-like protein 1), and Nab2p (nuclear polyadenylated RNA binding 2), were identified in a screen for proteins that cross-link to polyadenylated RNA  in vivo ( 26,  27).	bind
10622	1	3411	7	11	NULL	0	NULL	Pub1p	GP		crosslink to					RNA	NucleicAcid	polyadenylated			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_7752_s_48	11779864	(A)-binding protein 1), Pub1p (poly(U)-binding protein 1), Npl3p (nuclear protein localization 3), Hrp1p (hnRNP-like protein 1), and Nab2p (nuclear polyadenylated RNA binding 2), were identified in a screen for proteins that cross-link to polyadenylated RNA  in vivo ( 26,  27).	bind
10623	2	3411	7	11	NULL	0	NULL	Npl3p	GP		crosslink to					RNA	NucleicAcid	polyadenylated			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_7752_s_48	11779864	(A)-binding protein 1), Pub1p (poly(U)-binding protein 1), Npl3p (nuclear protein localization 3), Hrp1p (hnRNP-like protein 1), and Nab2p (nuclear polyadenylated RNA binding 2), were identified in a screen for proteins that cross-link to polyadenylated RNA  in vivo ( 26,  27).	bind
10624	3	3411	7	11	NULL	0	NULL	Hrp1p	GP		crosslink to					RNA	NucleicAcid	polyadenylated 			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_7752_s_48	11779864	(A)-binding protein 1), Pub1p (poly(U)-binding protein 1), Npl3p (nuclear protein localization 3), Hrp1p (hnRNP-like protein 1), and Nab2p (nuclear polyadenylated RNA binding 2), were identified in a screen for proteins that cross-link to polyadenylated RNA  in vivo ( 26,  27).	bind
10625	4	3411	7	11	NULL	0	NULL	Nab2p 	GP		crosslink to					RNA	NucleicAcid	polyadenylated			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_7752_s_48	11779864	(A)-binding protein 1), Pub1p (poly(U)-binding protein 1), Npl3p (nuclear protein localization 3), Hrp1p (hnRNP-like protein 1), and Nab2p (nuclear polyadenylated RNA binding 2), were identified in a screen for proteins that cross-link to polyadenylated RNA  in vivo ( 26,  27).	bind
10626	5	3411	7	11	NULL	0	NULL	Pub1p	GP		is					poly(U)-binding protein 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_7752_s_48	11779864	(A)-binding protein 1), Pub1p (poly(U)-binding protein 1), Npl3p (nuclear protein localization 3), Hrp1p (hnRNP-like protein 1), and Nab2p (nuclear polyadenylated RNA binding 2), were identified in a screen for proteins that cross-link to polyadenylated RNA  in vivo ( 26,  27).	bind
10629	6	3411	7	11	NULL	0	NULL	Npl3p	GP		is					nuclear protein localization 3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_7752_s_48	11779864	(A)-binding protein 1), Pub1p (poly(U)-binding protein 1), Npl3p (nuclear protein localization 3), Hrp1p (hnRNP-like protein 1), and Nab2p (nuclear polyadenylated RNA binding 2), were identified in a screen for proteins that cross-link to polyadenylated RNA  in vivo ( 26,  27).	bind
10634	7	3411	7	11	NULL	0	NULL	Hrp1p 	GP		is					hnRNP-like protein 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_7752_s_48	11779864	(A)-binding protein 1), Pub1p (poly(U)-binding protein 1), Npl3p (nuclear protein localization 3), Hrp1p (hnRNP-like protein 1), and Nab2p (nuclear polyadenylated RNA binding 2), were identified in a screen for proteins that cross-link to polyadenylated RNA  in vivo ( 26,  27).	bind
10636	8	3411	7	11	NULL	0	NULL	Nab2p	GP		is					nuclear polyadenylated RNA binding 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_7752_s_48	11779864	(A)-binding protein 1), Pub1p (poly(U)-binding protein 1), Npl3p (nuclear protein localization 3), Hrp1p (hnRNP-like protein 1), and Nab2p (nuclear polyadenylated RNA binding 2), were identified in a screen for proteins that cross-link to polyadenylated RNA  in vivo ( 26,  27).	bind
80538	1	3411	11	NULL	NULL	0	NULL	Pub1p	Protein		is					poly(U)-binding protein 1	Protein				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_10_7752_s_48	11779864	(A)-binding protein 1), Pub1p (poly(U)-binding protein 1), Npl3p (nuclear protein localization 3), Hrp1p (hnRNP-like protein 1), and Nab2p (nuclear polyadenylated RNA binding 2), were identified in a screen for proteins that cross-link to polyadenylated RNA  in vivo ( 26,  27).	bind
80539	2	3411	11	NULL	NULL	0	NULL	Npl3p	Protein		is					nuclear protein localization 3	Protein				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_10_7752_s_48	11779864	(A)-binding protein 1), Pub1p (poly(U)-binding protein 1), Npl3p (nuclear protein localization 3), Hrp1p (hnRNP-like protein 1), and Nab2p (nuclear polyadenylated RNA binding 2), were identified in a screen for proteins that cross-link to polyadenylated RNA  in vivo ( 26,  27).	bind
80540	3	3411	11	NULL	NULL	0	NULL	Hrp1p	Protein		is					hnRNP-like protein 1	Protein				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_10_7752_s_48	11779864	(A)-binding protein 1), Pub1p (poly(U)-binding protein 1), Npl3p (nuclear protein localization 3), Hrp1p (hnRNP-like protein 1), and Nab2p (nuclear polyadenylated RNA binding 2), were identified in a screen for proteins that cross-link to polyadenylated RNA  in vivo ( 26,  27).	bind
80541	4	3411	11	NULL	NULL	0	NULL	Nab2p	Protein		is					nuclear polyadenylated RNA binding 2	Protein				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_10_7752_s_48	11779864	(A)-binding protein 1), Pub1p (poly(U)-binding protein 1), Npl3p (nuclear protein localization 3), Hrp1p (hnRNP-like protein 1), and Nab2p (nuclear polyadenylated RNA binding 2), were identified in a screen for proteins that cross-link to polyadenylated RNA  in vivo ( 26,  27).	bind
80542	5	3411	11	NULL	NULL	0	NULL	Pub1p	Protein		cross-link to					RNA	NucleicAcidSubstance	polyadenylated			NULL	in vivo	0	NULL	NULL	NULL	gw60_jbiolchem_277_10_7752_s_48	11779864	(A)-binding protein 1), Pub1p (poly(U)-binding protein 1), Npl3p (nuclear protein localization 3), Hrp1p (hnRNP-like protein 1), and Nab2p (nuclear polyadenylated RNA binding 2), were identified in a screen for proteins that cross-link to polyadenylated RNA  in vivo ( 26,  27).	bind
80543	6	3411	11	NULL	NULL	0	NULL	Npl3p	Protein		cross-link to					RNA	NucleicAcidSubstance	polyadenylated			NULL	in vivo	0	NULL	NULL	NULL	gw60_jbiolchem_277_10_7752_s_48	11779864	(A)-binding protein 1), Pub1p (poly(U)-binding protein 1), Npl3p (nuclear protein localization 3), Hrp1p (hnRNP-like protein 1), and Nab2p (nuclear polyadenylated RNA binding 2), were identified in a screen for proteins that cross-link to polyadenylated RNA  in vivo ( 26,  27).	bind
80544	7	3411	11	NULL	NULL	0	NULL	Hrp1p	Protein		cross-link to					RNA	NucleicAcidSubstance	polyadenylated			NULL	in vivo	0	NULL	NULL	NULL	gw60_jbiolchem_277_10_7752_s_48	11779864	(A)-binding protein 1), Pub1p (poly(U)-binding protein 1), Npl3p (nuclear protein localization 3), Hrp1p (hnRNP-like protein 1), and Nab2p (nuclear polyadenylated RNA binding 2), were identified in a screen for proteins that cross-link to polyadenylated RNA  in vivo ( 26,  27).	bind
80545	8	3411	11	NULL	NULL	0	NULL	Nab2p	Protein		cross-link to					RNA	NucleicAcidSubstance	polyadenylated			NULL	in vivo	0	NULL	NULL	NULL	gw60_jbiolchem_277_10_7752_s_48	11779864	(A)-binding protein 1), Pub1p (poly(U)-binding protein 1), Npl3p (nuclear protein localization 3), Hrp1p (hnRNP-like protein 1), and Nab2p (nuclear polyadenylated RNA binding 2), were identified in a screen for proteins that cross-link to polyadenylated RNA  in vivo ( 26,  27).	bind
7564	1	3412	6	11	NULL	0	NULL	poly(A)-binding protein cytoplasmic 1	GP		is					PABPC1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_26_9773_s_137	16785428	(A)-binding protein cytoplasmic 1 (PABPC1) binds and colocalizes with paxillin, and disruption of this interaction inhibited cell migration ( ).	bind
7565	2	3412	6	11	NULL	0	NULL	PABPC1	GP		bind					paxillin	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_26_9773_s_137	16785428	(A)-binding protein cytoplasmic 1 (PABPC1) binds and colocalizes with paxillin, and disruption of this interaction inhibited cell migration ( ).	bind
7566	3	3412	6	11	NULL	0	NULL	PABPC1	GP		colocalizes with					paxillin	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_26_9773_s_137	16785428	(A)-binding protein cytoplasmic 1 (PABPC1) binds and colocalizes with paxillin, and disruption of this interaction inhibited cell migration ( ).	bind
7567	4	3412	6	11	NULL	0	NULL	statement 2	Process	disruption of	inhibits					cell migration	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_26_9773_s_137	16785428	(A)-binding protein cytoplasmic 1 (PABPC1) binds and colocalizes with paxillin, and disruption of this interaction inhibited cell migration ( ).	bind
10637	1	3412	7	11	NULL	0	NULL	PABPC1	GP		bind					paxillin	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_26_9773_s_137	16785428	(A)-binding protein cytoplasmic 1 (PABPC1) binds and colocalizes with paxillin, and disruption of this interaction inhibited cell migration ( ).	bind
10639	2	3412	7	11	NULL	0	NULL	PABPC1	GP		colocalizes with					paxillin	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_26_9773_s_137	16785428	(A)-binding protein cytoplasmic 1 (PABPC1) binds and colocalizes with paxillin, and disruption of this interaction inhibited cell migration ( ).	bind
10640	3	3412	7	11	NULL	0	NULL	statement 1	Process	disruption of	inhibits					cell migration	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_26_9773_s_137	16785428	(A)-binding protein cytoplasmic 1 (PABPC1) binds and colocalizes with paxillin, and disruption of this interaction inhibited cell migration ( ).	bind
80546	1	3412	11	NULL	NULL	0	NULL	PABPC1	Protein		binds to 					paxillin	Protein				NULL		0	NULL	NULL	NULL	gw70_pnas_103_26_9773_s_137	16785428	(A)-binding protein cytoplasmic 1 (PABPC1) binds and colocalizes with paxillin, and disruption of this interaction inhibited cell migration ( ).	bind
80547	2	3412	11	NULL	NULL	0	NULL	PABPC1	Protein		colocalizes with					paxillin	Protein				NULL		0	NULL	NULL	NULL	gw70_pnas_103_26_9773_s_137	16785428	(A)-binding protein cytoplasmic 1 (PABPC1) binds and colocalizes with paxillin, and disruption of this interaction inhibited cell migration ( ).	bind
80548	3	3412	11	NULL	NULL	0	NULL	statement 1	Process		occurs along with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_103_26_9773_s_137	16785428	(A)-binding protein cytoplasmic 1 (PABPC1) binds and colocalizes with paxillin, and disruption of this interaction inhibited cell migration ( ).	bind
80549	4	3412	11	NULL	NULL	0	NULL	statement 1	Process	disruption of	inhibit					cell migration	BiologicalProcess				NULL		0	NULL	NULL	NULL	gw70_pnas_103_26_9773_s_137	16785428	(A)-binding protein cytoplasmic 1 (PABPC1) binds and colocalizes with paxillin, and disruption of this interaction inhibited cell migration ( ).	bind
7568	1	3413	6	11	NULL	0	NULL	Pab1p	GP		bind					eIF4F	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_13_4107_s_219	9233819	(A)-binding protein Pab1p which binds eIF4F only in the presence of poly	bind
10641	1	3413	7	11	NULL	0	NULL	Pab1p	GP		bind					eIF4F	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_13_4107_s_219	9233819	(A)-binding protein Pab1p which binds eIF4F only in the presence of poly	bind
80550	1	3413	11	NULL	NULL	0	NULL	 Pab1p	Protein		binds to 					eIF4F	Protein				NULL		0	NULL	NULL	NULL	gw60_embo_16_13_4107_s_219	9233819	(A)-binding protein Pab1p which binds eIF4F only in the presence of poly	bind
7571	1	3414	6	11	NULL	0	NULL	poly(A)-binding protein	GP		is					Pab1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_62_4_1492_s_252	9841679	(A)-binding protein Pab1p, are also found associated with the eIF4F components of  S. cerevisiae; p20 competes with eIF4G for binding to eIF4E, and Pab1p binds to eIF4F via a site on eIF4G ( 10,  15,  539).	bind
7572	2	3414	6	11	NULL	0	NULL	Pab1p	GP		bind					eIF4F	GP	S. cerevisiae			NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_62_4_1492_s_252	9841679	(A)-binding protein Pab1p, are also found associated with the eIF4F components of  S. cerevisiae; p20 competes with eIF4G for binding to eIF4E, and Pab1p binds to eIF4F via a site on eIF4G ( 10,  15,  539).	bind
7573	3	3414	6	11	NULL	0	NULL	statement 2	Process		occurs via					eIF4G	GP				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_62_4_1492_s_252	9841679	(A)-binding protein Pab1p, are also found associated with the eIF4F components of  S. cerevisiae; p20 competes with eIF4G for binding to eIF4E, and Pab1p binds to eIF4F via a site on eIF4G ( 10,  15,  539).	bind
7574	4	3414	6	11	NULL	0	NULL	eIF4E	GP		bind					eIF4G	GP				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_62_4_1492_s_252	9841679	(A)-binding protein Pab1p, are also found associated with the eIF4F components of  S. cerevisiae; p20 competes with eIF4G for binding to eIF4E, and Pab1p binds to eIF4F via a site on eIF4G ( 10,  15,  539).	bind
7575	5	3414	6	11	NULL	0	NULL	p20	GP		bind					eIF4G	GP				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_62_4_1492_s_252	9841679	(A)-binding protein Pab1p, are also found associated with the eIF4F components of  S. cerevisiae; p20 competes with eIF4G for binding to eIF4E, and Pab1p binds to eIF4F via a site on eIF4G ( 10,  15,  539).	bind
7576	6	3414	6	11	NULL	0	NULL	statement 4	GP		competes					statement 5	GP				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_62_4_1492_s_252	9841679	(A)-binding protein Pab1p, are also found associated with the eIF4F components of  S. cerevisiae; p20 competes with eIF4G for binding to eIF4E, and Pab1p binds to eIF4F via a site on eIF4G ( 10,  15,  539).	bind
10645	1	3414	7	11	NULL	0	NULL	p20	GP		bind					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_62_4_1492_s_252	9841679	(A)-binding protein Pab1p, are also found associated with the eIF4F components of  S. cerevisiae; p20 competes with eIF4G for binding to eIF4E, and Pab1p binds to eIF4F via a site on eIF4G ( 10,  15,  539).	bind
10646	2	3414	7	11	NULL	0	NULL	eIF4G	GP		bind					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_62_4_1492_s_252	9841679	(A)-binding protein Pab1p, are also found associated with the eIF4F components of  S. cerevisiae; p20 competes with eIF4G for binding to eIF4E, and Pab1p binds to eIF4F via a site on eIF4G ( 10,  15,  539).	bind
10648	3	3414	7	11	NULL	0	NULL	statement 1	Process		compete with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_62_4_1492_s_252	9841679	(A)-binding protein Pab1p, are also found associated with the eIF4F components of  S. cerevisiae; p20 competes with eIF4G for binding to eIF4E, and Pab1p binds to eIF4F via a site on eIF4G ( 10,  15,  539).	bind
10649	4	3414	7	11	NULL	0	NULL	Pab1p	GP		bind					eIF4F	GP	S. cerevisiae			NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_62_4_1492_s_252	9841679	(A)-binding protein Pab1p, are also found associated with the eIF4F components of  S. cerevisiae; p20 competes with eIF4G for binding to eIF4E, and Pab1p binds to eIF4F via a site on eIF4G ( 10,  15,  539).	bind
10651	5	3414	7	11	NULL	0	NULL	statement 4	Process		occurs via					eIF4G	GP				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_62_4_1492_s_252	9841679	(A)-binding protein Pab1p, are also found associated with the eIF4F components of  S. cerevisiae; p20 competes with eIF4G for binding to eIF4E, and Pab1p binds to eIF4F via a site on eIF4G ( 10,  15,  539).	bind
80551	1	3414	11	NULL	NULL	0	NULL	Pab1p	Protein		associated with					eIF4F 	Protein	S. cerevisiae			NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_62_4_1492_s_252	9841679	(A)-binding protein Pab1p, are also found associated with the eIF4F components of  S. cerevisiae; p20 competes with eIF4G for binding to eIF4E, and Pab1p binds to eIF4F via a site on eIF4G ( 10,  15,  539).	bind
80552	2	3414	11	NULL	NULL	0	NULL	p20	Protein		competes with					eIF4G	Protein				NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_62_4_1492_s_252	9841679	(A)-binding protein Pab1p, are also found associated with the eIF4F components of  S. cerevisiae; p20 competes with eIF4G for binding to eIF4E, and Pab1p binds to eIF4F via a site on eIF4G ( 10,  15,  539).	bind
80553	3	3414	11	NULL	NULL	0	NULL	p20	Protein		binds to 					eIF4E	Protein				NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_62_4_1492_s_252	9841679	(A)-binding protein Pab1p, are also found associated with the eIF4F components of  S. cerevisiae; p20 competes with eIF4G for binding to eIF4E, and Pab1p binds to eIF4F via a site on eIF4G ( 10,  15,  539).	bind
80554	4	3414	11	NULL	NULL	0	NULL	eIF4G	Protein		binds to 					eIF4E	Protein				NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_62_4_1492_s_252	9841679	(A)-binding protein Pab1p, are also found associated with the eIF4F components of  S. cerevisiae; p20 competes with eIF4G for binding to eIF4E, and Pab1p binds to eIF4F via a site on eIF4G ( 10,  15,  539).	bind
80555	5	3414	11	NULL	NULL	0	NULL	statement 1	Process		occurs via					eIF4G	Protein				NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_62_4_1492_s_252	9841679	(A)-binding protein Pab1p, are also found associated with the eIF4F components of  S. cerevisiae; p20 competes with eIF4G for binding to eIF4E, and Pab1p binds to eIF4F via a site on eIF4G ( 10,  15,  539).	bind
7579	1	3415	6	11	NULL	0	NULL	Xenopus-specific protein	GP		bind									AU-rich sequences	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_2060_s_91	15713657	(A)-binding protein was identified as a  Xenopus-specific protein that binds AU-rich sequences ( ).	bind
10652	1	3415	7	11	NULL	0	NULL	Xenopus-specific protein	GP		bind									AU-rich sequences	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_2060_s_91	15713657	(A)-binding protein was identified as a  Xenopus-specific protein that binds AU-rich sequences ( ).	bind
80556	1	3415	11	NULL	NULL	0	NULL	protein	Protein	Xenopus-specific	binds to 					AU-rich sequence	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_5_2060_s_91	15713657	(A)-binding protein was identified as a  Xenopus-specific protein that binds AU-rich sequences ( ).	bind
7581	2	3418	6	11	NULL	0	NULL	eIF4B	GP		does not bind					Hsp27	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_12_1460_s_8	10859165	(A)-binding protein, eIF4B, and eIF3 were not bound by Hsp27 and were not recruited into insoluble complexes.	bind
7582	3	3418	6	11	NULL	0	NULL	eIF3	GP		does not bind					Hsp27	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_12_1460_s_8	10859165	(A)-binding protein, eIF4B, and eIF3 were not bound by Hsp27 and were not recruited into insoluble complexes.	bind
7584	5	3418	6	11	NULL	0	NULL	eIF4B	GP		are not recruited into					insoluble complexes	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_12_1460_s_8	10859165	(A)-binding protein, eIF4B, and eIF3 were not bound by Hsp27 and were not recruited into insoluble complexes.	bind
7585	6	3418	6	11	NULL	0	NULL	eIF3	GP		are not recruited into					insoluble complexes	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_12_1460_s_8	10859165	(A)-binding protein, eIF4B, and eIF3 were not bound by Hsp27 and were not recruited into insoluble complexes.	bind
10654	1	3418	7	11	NULL	0	NULL	eIF4B	GP		does not bind					Hsp27	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_12_1460_s_8	10859165	(A)-binding protein, eIF4B, and eIF3 were not bound by Hsp27 and were not recruited into insoluble complexes.	bind
10655	2	3418	7	11	NULL	0	NULL	 eIF3	GP		does not bind					Hsp27	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_12_1460_s_8	10859165	(A)-binding protein, eIF4B, and eIF3 were not bound by Hsp27 and were not recruited into insoluble complexes.	bind
10657	3	3418	7	11	NULL	0	NULL	 eIF4B	GP		is not recruited into					insoluble complexes	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_12_1460_s_8	10859165	(A)-binding protein, eIF4B, and eIF3 were not bound by Hsp27 and were not recruited into insoluble complexes.	bind
10658	4	3418	7	11	NULL	0	NULL	eIF3	GP		is not recruited into					insoluble complexes	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_12_1460_s_8	10859165	(A)-binding protein, eIF4B, and eIF3 were not bound by Hsp27 and were not recruited into insoluble complexes.	bind
80557	1	3418	11	NULL	NULL	0	NULL	eIF4B	Protein		not bind to					Hsp27	Protein				NULL		0	NULL	NULL	NULL	gw60_genesdev_14_12_1460_s_8	10859165	(A)-binding protein, eIF4B, and eIF3 were not bound by Hsp27 and were not recruited into insoluble complexes.	bind
80558	2	3418	11	NULL	NULL	0	NULL	eIF3	Protein		not bind to 					Hsp27	Protein				NULL		0	NULL	NULL	NULL	gw60_genesdev_14_12_1460_s_8	10859165	(A)-binding protein, eIF4B, and eIF3 were not bound by Hsp27 and were not recruited into insoluble complexes.	bind
7587	2	3421	6	11	NULL	0	NULL	PARN	GP		bind 									EDEN sequence	NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_35_0_365_s_98	11700288	(A)-specific RNase (PARN) ( 100) and EDEN-BP ( 162), which binds to the EDEN sequence.	bind
7588	3	3421	6	11	NULL	0	NULL	EDEN-BP	GP		bind									EDEN sequence	NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_35_0_365_s_98	11700288	(A)-specific RNase (PARN) ( 100) and EDEN-BP ( 162), which binds to the EDEN sequence.	bind
10659	1	3421	7	11	NULL	0	NULL	PARN	GP		bind									EDEN sequence	NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_35_0_365_s_98	11700288	(A)-specific RNase (PARN) ( 100) and EDEN-BP ( 162), which binds to the EDEN sequence.	bind
10660	2	3421	7	11	NULL	0	NULL	EDEN-BP	GP		bind									EDEN sequence	NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_35_0_365_s_98	11700288	(A)-specific RNase (PARN) ( 100) and EDEN-BP ( 162), which binds to the EDEN sequence.	bind
80559	1	3421	11	NULL	NULL	0	NULL	PARN	Protein		binds to 					EDEN sequence	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_annurevgenet_35_0_365_s_98	11700288	(A)-specific RNase (PARN) ( 100) and EDEN-BP ( 162), which binds to the EDEN sequence.	bind
80560	2	3421	11	NULL	NULL	0	NULL	EDEN-BP	Protein		binds to 					EDEN sequence	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_annurevgenet_35_0_365_s_98	11700288	(A)-specific RNase (PARN) ( 100) and EDEN-BP ( 162), which binds to the EDEN sequence.	bind
7589	1	3422	6	11	NULL	0	NULL	poly(A)-tail-induced initiation factor 	GP		bind					m7G cap	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_1_104_s_163	15630022	(A)-tail-induced initiation factor binding to the m7G cap.	bind
10661	1	3422	7	11	NULL	0	NULL	poly(A)-tail-induced initiation factor	GP		bind					m7G cap	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_1_104_s_163	15630022	(A)-tail-induced initiation factor binding to the m7G cap.	bind
80561	1	3422	11	NULL	NULL	0	NULL	initiation factor	Protein		binds to 					m7G cap	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_1_104_s_163	15630022	(A)-tail-induced initiation factor binding to the m7G cap.	bind
7590	1	3423	6	11	NULL	0	NULL	NC	GP		bind									(TG)4	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_2_472_s_300	16434700	(A)30 (open squares) or (TG)10 (open triangles), was able to completely prevent the binding of NC to (TG)4 on the SPR surface (i.e. the ISmin was 0, as indicated in  Table 3).	bind
7591	2	3423	6	11	NULL	0	NULL				prevents				(TG)10	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_2_472_s_300	16434700	(A)30 (open squares) or (TG)10 (open triangles), was able to completely prevent the binding of NC to (TG)4 on the SPR surface (i.e. the ISmin was 0, as indicated in  Table 3).	bind
10663	1	3423	7	11	NULL	0	NULL	NC 	GP		bind									(TG)4	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_2_472_s_300	16434700	(A)30 (open squares) or (TG)10 (open triangles), was able to completely prevent the binding of NC to (TG)4 on the SPR surface (i.e. the ISmin was 0, as indicated in  Table 3).	bind
10664	2	3423	7	11	NULL	0	NULL				prevent				(TG)10	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_2_472_s_300	16434700	(A)30 (open squares) or (TG)10 (open triangles), was able to completely prevent the binding of NC to (TG)4 on the SPR surface (i.e. the ISmin was 0, as indicated in  Table 3).	bind
80562	1	3423	11	NULL	NULL	0	NULL	NC	Chemical		binds to 					(TG)4	NucleicAcidSubstance	SPR surface			NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_34_2_472_s_300	16434700	(A)30 (open squares) or (TG)10 (open triangles), was able to completely prevent the binding of NC to (TG)4 on the SPR surface (i.e. the ISmin was 0, as indicated in  Table 3).	bind
7632	1	3424	6	11	NULL	0	NULL	NC	GP		bind									(TG)4	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_2_472_s_259	16434700	(A)30 completely eliminated binding of NC to (TG)4, as expected.	bind
10666	1	3424	7	11	NULL	0	NULL	NC	GP		bind									(TG)4	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_2_472_s_259	16434700	(A)30 completely eliminated binding of NC to (TG)4, as expected.	bind
80563	1	3424	11	NULL	NULL	0	NULL	NC 	Chemical		binds to 					(TG)4	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_34_2_472_s_259	16434700	(A)30 completely eliminated binding of NC to (TG)4, as expected.	bind
7634	1	3426	6	11	NULL	0	NULL	RNA	NucleicAcid	radioactively labeled	bind				ARS	PABP	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_248	16356927	(A)50 RNA ( Figure 2C, lanes 9 - 14 and legend crosses in  Figure 2D) to attain a similar level of inhibition of the binding of radioactively labeled ARS RNA to PABP.	bind
7635	2	3426	6	11	NULL	0	NULL	50 RNA	NucleicAcid		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_248	16356927	(A)50 RNA ( Figure 2C, lanes 9 - 14 and legend crosses in  Figure 2D) to attain a similar level of inhibition of the binding of radioactively labeled ARS RNA to PABP.	bind
10686	1	3426	7	11	NULL	0	NULL	PABP	GP		bind					RNA	NucleicAcid	radioactively labeled		ARS	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_248	16356927	(A)50 RNA ( Figure 2C, lanes 9 - 14 and legend crosses in  Figure 2D) to attain a similar level of inhibition of the binding of radioactively labeled ARS RNA to PABP.	bind
14953	2	3426	7	11	NULL	0	NULL	50 RNA	NucleicAcid		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_248	16356927	(A)50 RNA ( Figure 2C, lanes 9 - 14 and legend crosses in  Figure 2D) to attain a similar level of inhibition of the binding of radioactively labeled ARS RNA to PABP.	bind
80564	1	3426	11	NULL	NULL	0	NULL	ARS RNA	NucleicAcidSubstance	radioactively labeled	inhibit					PABP	Protein				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_248	16356927	(A)50 RNA ( Figure 2C, lanes 9 - 14 and legend crosses in  Figure 2D) to attain a similar level of inhibition of the binding of radioactively labeled ARS RNA to PABP.	bind
7636	1	3427	6	11	NULL	0	NULL	IMP1	GP		bind					RNA	NucleicAcid	labeled		ARS	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_294	16356927	(A)50 RNA competed with the binding of both 63 (IMP1) and 105 (UNR) kDa polypeptides to the labeled ARS RNA.	bind
7637	2	3427	6	11	NULL	0	NULL	50 RNA	NucleicAcid		bind					RNA	NucleicAcid	labeled		ARS	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_294	16356927	(A)50 RNA competed with the binding of both 63 (IMP1) and 105 (UNR) kDa polypeptides to the labeled ARS RNA.	bind
7638	3	3427	6	11	NULL	0	NULL	statement 1	GP		competes					statement 2	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_294	16356927	(A)50 RNA competed with the binding of both 63 (IMP1) and 105 (UNR) kDa polypeptides to the labeled ARS RNA.	bind
7639	4	3427	6	10	NULL	0	NULL	UNR	NULL		bind	NULL				RNA	NULL	labeled		ARS	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_294	16356927	(A)50 RNA competed with the binding of both 63 (IMP1) and 105 (UNR) kDa polypeptides to the labeled ARS RNA.	bind
7641	5	3427	6	10	NULL	0	NULL	statement 4	NULL		competes	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_294	16356927	(A)50 RNA competed with the binding of both 63 (IMP1) and 105 (UNR) kDa polypeptides to the labeled ARS RNA.	bind
10687	1	3427	7	11	NULL	0	NULL	IMP1 polypeptide	GP		bind					 RNA	NucleicAcid	labeled		ARS	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_294	16356927	(A)50 RNA competed with the binding of both 63 (IMP1) and 105 (UNR) kDa polypeptides to the labeled ARS RNA.	bind
10688	2	3427	7	11	NULL	0	NULL	UNR polypeptide	GP		bind					 RNA	NucleicAcid	labeled		ARS	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_294	16356927	(A)50 RNA competed with the binding of both 63 (IMP1) and 105 (UNR) kDa polypeptides to the labeled ARS RNA.	bind
14958	5	3427	7	11	NULL	0	NULL	50 RNA	NucleicAcid		bind					 RNA	NucleicAcid			ARS	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_294	16356927	(A)50 RNA competed with the binding of both 63 (IMP1) and 105 (UNR) kDa polypeptides to the labeled ARS RNA.	bind
14959	6	3427	7	11	NULL	0	NULL	statement 5	NucleicAcid		compete with					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_294	16356927	(A)50 RNA competed with the binding of both 63 (IMP1) and 105 (UNR) kDa polypeptides to the labeled ARS RNA.	bind
14960	7	3427	7	11	NULL	0	NULL	statement 5	NucleicAcid		compete with					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_294	16356927	(A)50 RNA competed with the binding of both 63 (IMP1) and 105 (UNR) kDa polypeptides to the labeled ARS RNA.	bind
80565	1	3427	11	NULL	NULL	0	NULL	poly(A)50 RNA	NucleicAcidSubstance		competes with					IMP1 polypeptide	PartOfProtein				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_294	16356927	(A)50 RNA competed with the binding of both 63 (IMP1) and 105 (UNR) kDa polypeptides to the labeled ARS RNA.	bind
80566	2	3427	11	NULL	NULL	0	NULL	poly(A)50 RNA	NucleicAcidSubstance		competes with					UNR polypeptide	PartOfProtein				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_294	16356927	(A)50 RNA competed with the binding of both 63 (IMP1) and 105 (UNR) kDa polypeptides to the labeled ARS RNA.	bind
80567	3	3427	11	NULL	NULL	0	NULL	poly(A)50 RNA	NucleicAcidSubstance		binds to 					ARS RNA	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_294	16356927	(A)50 RNA competed with the binding of both 63 (IMP1) and 105 (UNR) kDa polypeptides to the labeled ARS RNA.	bind
80568	4	3427	11	NULL	NULL	0	NULL	IMP1 polypeptide	PartOfProtein		binds to 					ARS RNA	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_294	16356927	(A)50 RNA competed with the binding of both 63 (IMP1) and 105 (UNR) kDa polypeptides to the labeled ARS RNA.	bind
80569	5	3427	11	NULL	NULL	0	NULL	UNR polypeptide	PartOfProtein		binds to 					ARS RNA	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_294	16356927	(A)50 RNA competed with the binding of both 63 (IMP1) and 105 (UNR) kDa polypeptides to the labeled ARS RNA.	bind
80570	1	3428	11	NULL	NULL	0	NULL	NF-IL-6	Protein		contain					 palindrome	NucleicAcidSubstance			CCTTGCTGCAAGG	NULL		0	NULL	NULL	NULL	gw60_gene_237_1_177_s_66	10524248	(A); a palindrome (CCTTGCTGCAAGG) containing NF-IL-6 and GAS-like elements (P); two IRF-1-like sites (I1 and I2); an Ets-1 binding motif (E); and an ISRE.	bind
7642	1	3430	6	11	NULL	0	NULL	GDP	Chemical		bind					Rab11A	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_8_3530_s_149	15181150	(A); with the GDP-bound  form of Rab11A (C); and with the GppNHp-bound form of Rab4B (D).	bind
7644	2	3430	6	11	NULL	0	NULL	GppNHp	Chemical		bind					Rab4B	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_8_3530_s_149	15181150	(A); with the GDP-bound  form of Rab11A (C); and with the GppNHp-bound form of Rab4B (D).	bind
10689	1	3430	7	11	NULL	0	NULL	GDP	Chemical		bind					Rab11A	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_8_3530_s_149	15181150	(A); with the GDP-bound  form of Rab11A (C); and with the GppNHp-bound form of Rab4B (D).	bind
10690	2	3430	7	11	NULL	0	NULL	GppNHp	Chemical		bind					Rab4B	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_8_3530_s_149	15181150	(A); with the GDP-bound  form of Rab11A (C); and with the GppNHp-bound form of Rab4B (D).	bind
80571	1	3430	11	NULL	NULL	0	NULL	Rab11A	Protein		binds to 					 GDP	Chemical				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_8_3530_s_149	15181150	(A); with the GDP-bound  form of Rab11A (C); and with the GppNHp-bound form of Rab4B (D).	bind
80572	2	3430	11	NULL	NULL	0	NULL	Rab4B	Protein		binds to 					GppNHp	Chemical				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_8_3530_s_149	15181150	(A); with the GDP-bound  form of Rab11A (C); and with the GppNHp-bound form of Rab4B (D).	bind
7649	1	3431	6	11	NULL	0	NULL	eukaryotic initiation factor 4F	GP		bind					cap analogues	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_16_4372_s_507	10944120	(A)binding protein enhances the binding affinity of eukaryotic initiation factor 4F and (iso)4F for cap analogues.	bind
7651	2	3431	6	11	NULL	0	NULL	eukaryotic initiation factor (iso)4F	GP		bind					cap analogues	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_16_4372_s_507	10944120	(A)binding protein enhances the binding affinity of eukaryotic initiation factor 4F and (iso)4F for cap analogues.	bind
10691	1	3431	7	11	NULL	0	NULL	 eukaryotic initiation factor 4F	GP		bind					cap analogues	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_16_4372_s_507	10944120	(A)binding protein enhances the binding affinity of eukaryotic initiation factor 4F and (iso)4F for cap analogues.	bind
10694	2	3431	7	11	NULL	0	NULL	eukaryotic initiation factor (iso)4F	GP		bind					cap analogues	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_16_4372_s_507	10944120	(A)binding protein enhances the binding affinity of eukaryotic initiation factor 4F and (iso)4F for cap analogues.	bind
80573	1	3431	11	NULL	NULL	0	NULL	poly(A)binding protein 	Protein		binds to 		enhances			eukaryotic initiation factor 4F	Protein				NULL		0	NULL	NULL	NULL	gw60_embo_19_16_4372_s_507	10944120	(A)binding protein enhances the binding affinity of eukaryotic initiation factor 4F and (iso)4F for cap analogues.	bind
80574	1	3432	11	NULL	NULL	0	NULL	GABAAR &#946;3	Protein	dephosphorylated	binds to 		high affinity			AP2	Protein				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_proc-natl-acad-sci-u-s-a_102_41_16192353_s_10	16192353	(A)R beta3 subunit binds  to AP2 with high affinity only when dephosphorylated.	bind
7657	1	3435	6	11	NULL	0	NULL				bind				S-TATA composite box	GTFs	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_3_834_s_121	10629040	(A)S-TATA composite box binds GTFs.	bind
10701	1	3435	7	11	NULL	0	NULL				binds				S-TATA composite box	GTFs	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_3_834_s_121	10629040	(A)S-TATA composite box binds GTFs.	bind
7658	1	3436	6	11	NULL	0	NULL				does not bind		efficiently		S-TATA	TBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_3_834_s_127	10629040	(A)S-TATA does not bind TBP efficiently (lane 1) but binds the mixture of the three GTF proteins (lane 7).	bind
7659	2	3436	6	11	NULL	0	NULL				bind				S-TATA	GTF proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_3_834_s_127	10629040	(A)S-TATA does not bind TBP efficiently (lane 1) but binds the mixture of the three GTF proteins (lane 7).	bind
10702	1	3436	7	11	NULL	0	NULL				does not bind		efficiently		S-TATA	TBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_3_834_s_127	10629040	(A)S-TATA does not bind TBP efficiently (lane 1) but binds the mixture of the three GTF proteins (lane 7).	bind
10703	2	3436	7	11	NULL	0	NULL				bind				S-TATA	GTF proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_3_834_s_127	10629040	(A)S-TATA does not bind TBP efficiently (lane 1) but binds the mixture of the three GTF proteins (lane 7).	bind
80575	1	3436	11	NULL	NULL	0	NULL	P(A)S-TATA	NucleicAcidSubstance		does not bind to					TBP	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_3_834_s_127	10629040	(A)S-TATA does not bind TBP efficiently (lane 1) but binds the mixture of the three GTF proteins (lane 7).	bind
80576	2	3436	11	NULL	NULL	0	NULL	P(A)S-TATA	NucleicAcidSubstance		binds to 					GTF proteins	Protein	mixture			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_3_834_s_127	10629040	(A)S-TATA does not bind TBP efficiently (lane 1) but binds the mixture of the three GTF proteins (lane 7).	bind
7661	1	3437	6	11	NULL	0	NULL				bind				s-TATA	GTFs	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_3_834_s_154	10629040	(A)S-TATA sequence binds the GTFs in a manner genuinely characteristic of a promoter.	bind
7662	2	3437	6	11	NULL	0	NULL	statement 1	Process		is characteristic of									promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_3_834_s_154	10629040	(A)S-TATA sequence binds the GTFs in a manner genuinely characteristic of a promoter.	bind
10704	1	3437	7	11	NULL	0	NULL				binds				S-TATA sequence	GTFs	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_3_834_s_154	10629040	(A)S-TATA sequence binds the GTFs in a manner genuinely characteristic of a promoter.	bind
14965	2	3437	7	11	NULL	0	NULL	statement 1	Process		is characteristic of									promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_3_834_s_154	10629040	(A)S-TATA sequence binds the GTFs in a manner genuinely characteristic of a promoter.	bind
7698	1	3439	6	11	NULL	0	NULL	SH-SY5Y-h 7 cells	Cell	transfected	overexpress					7 receptors	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_13_2533_s_113	11044725	(A)] and saturation 125I- BTx binding [ Fig. 4(B)] to transfected SH-SY5Y-h 7 neuroblastoma cells overexpressing human  7 receptors also were consistent with a non-competitive mechanism of functional block by diltiazem.	bind
7699	2	3439	6	11	NULL	0	NULL	BTx	Chemical	125I-labeled	bind					statement 1	Cell				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_13_2533_s_113	11044725	(A)] and saturation 125I- BTx binding [ Fig. 4(B)] to transfected SH-SY5Y-h 7 neuroblastoma cells overexpressing human  7 receptors also were consistent with a non-competitive mechanism of functional block by diltiazem.	bind
52812	3	3439	6	11	NULL	0	NULL	SH-SY5Y-h 7 cells	Cell		is a type of					neuroblastoma cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_13_2533_s_113	11044725	(A)] and saturation 125I- BTx binding [ Fig. 4(B)] to transfected SH-SY5Y-h 7 neuroblastoma cells overexpressing human  7 receptors also were consistent with a non-competitive mechanism of functional block by diltiazem.	bind
10730	1	3439	7	11	NULL	0	NULL	BTx	Chemical	125I-labeled	bind					SH-SY5Y-h 7 cells	Cell	transfected			NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_13_2533_s_113	11044725	(A)] and saturation 125I- BTx binding [ Fig. 4(B)] to transfected SH-SY5Y-h 7 neuroblastoma cells overexpressing human  7 receptors also were consistent with a non-competitive mechanism of functional block by diltiazem.	bind
11753	2	3439	7	11	NULL	0	NULL	SH-SY5Y-h 7 cells	Cell	transfected	overexpress					7 receptors	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_13_2533_s_113	11044725	(A)] and saturation 125I- BTx binding [ Fig. 4(B)] to transfected SH-SY5Y-h 7 neuroblastoma cells overexpressing human  7 receptors also were consistent with a non-competitive mechanism of functional block by diltiazem.	bind
52813	3	3439	7	11	NULL	0	NULL	SH-SY5Y-h 7 cells	Cell		is a type of					neuroblastoma cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_13_2533_s_113	11044725	(A)] and saturation 125I- BTx binding [ Fig. 4(B)] to transfected SH-SY5Y-h 7 neuroblastoma cells overexpressing human  7 receptors also were consistent with a non-competitive mechanism of functional block by diltiazem.	bind
7663	1	3441	6	11	NULL	0	NULL	Ang IV	GP	125I-labeled	bind					MDBK cell membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_113	10565848	(A,  n = 4) and dithiothreitol (B,  n = 3) on 125I-Ang IV and 125I-divalinal Ang IV binding to MDBK cell membranes and 125I-Ang II binding to rat liver membranes.	bind
7664	2	3441	6	11	NULL	0	NULL	divalinal Ang IV	GP	125I-labeled	bind					MDBK cell membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_113	10565848	(A,  n = 4) and dithiothreitol (B,  n = 3) on 125I-Ang IV and 125I-divalinal Ang IV binding to MDBK cell membranes and 125I-Ang II binding to rat liver membranes.	bind
7665	3	3441	6	11	NULL	0	NULL	Ang II	GP	125I-labeled	bind					liver membranes	OrganismPart	rat			NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_113	10565848	(A,  n = 4) and dithiothreitol (B,  n = 3) on 125I-Ang IV and 125I-divalinal Ang IV binding to MDBK cell membranes and 125I-Ang II binding to rat liver membranes.	bind
10731	1	3441	7	11	NULL	0	NULL	divalinal Ang IV	GP	125I-labeled	bind					MDBK cell membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_113	10565848	(A,  n = 4) and dithiothreitol (B,  n = 3) on 125I-Ang IV and 125I-divalinal Ang IV binding to MDBK cell membranes and 125I-Ang II binding to rat liver membranes.	bind
10732	2	3441	7	11	NULL	0	NULL	Ang II	GP	125I-labeled	bind					liver membrane	OrganismPart	rat			NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_113	10565848	(A,  n = 4) and dithiothreitol (B,  n = 3) on 125I-Ang IV and 125I-divalinal Ang IV binding to MDBK cell membranes and 125I-Ang II binding to rat liver membranes.	bind
52814	3	3441	7	11	NULL	0	NULL	Ang IV	GP	125I-labeled	bind					MDBK cell membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_113	10565848	(A,  n = 4) and dithiothreitol (B,  n = 3) on 125I-Ang IV and 125I-divalinal Ang IV binding to MDBK cell membranes and 125I-Ang II binding to rat liver membranes.	bind
80577	1	3441	11	NULL	NULL	0	NULL	125I-Ang II	Protein		binds to 					membrane	CellComponent	rat liver			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_113	10565848	(A,  n = 4) and dithiothreitol (B,  n = 3) on 125I-Ang IV and 125I-divalinal Ang IV binding to MDBK cell membranes and 125I-Ang II binding to rat liver membranes.	bind
80578	2	3441	11	NULL	NULL	0	NULL	125I-divalinal Ang IV	Protein		binds to 					cell membrane	CellComponent	MDBK			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_113	10565848	(A,  n = 4) and dithiothreitol (B,  n = 3) on 125I-Ang IV and 125I-divalinal Ang IV binding to MDBK cell membranes and 125I-Ang II binding to rat liver membranes.	bind
80579	3	3441	11	NULL	NULL	0	NULL	125I-Ang IV	Protein		binds to 					cell membrane	CellComponent	MDBK			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_113	10565848	(A,  n = 4) and dithiothreitol (B,  n = 3) on 125I-Ang IV and 125I-divalinal Ang IV binding to MDBK cell membranes and 125I-Ang II binding to rat liver membranes.	bind
80580	1	3445	11	NULL	NULL	0	NULL	GST-fused protein	Protein		binds to 					glutathione-Sepharose 4B	PartOfProtein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_6_2242_s_300	15743821	(A, B, D, and E) The indicated [35]methionine-labeled products in vitro translated in rabbit reticulocyte lysates were  incubated with the different GST-fused proteins bound to glutathione-Sepharose 4B.	bind
7666	1	3447	6	11	NULL	0	NULL	TetR-GFP	GP		bind									TetO repeats	NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_4_1_55_s_172	15643060	(A, C, and E) and  TetR-GFP bound to  TetO repeats (B, D, and F) were visualized by fluorescence microscopy with UV and fluorescein  isothiocyanate optics, respectively.	bind
10733	1	3447	7	11	NULL	0	NULL	TetR-GFP	GP		bind									TetO repeats	NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_4_1_55_s_172	15643060	(A, C, and E) and  TetR-GFP bound to  TetO repeats (B, D, and F) were visualized by fluorescence microscopy with UV and fluorescein  isothiocyanate optics, respectively.	bind
80581	1	3447	11	NULL	NULL	0	NULL	TetR-GFP	PartOfProtein		binds to 					TetO repeats	PartOfProtein				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_1_55_s_172	15643060	(A, C, and E) and  TetR-GFP bound to  TetO repeats (B, D, and F) were visualized by fluorescence microscopy with UV and fluorescein  isothiocyanate optics, respectively.	bind
7667	1	3448	6	11	NULL	0	NULL	MAb 1E5 	GP		bind					PvpA	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_71_3_1265_s_143	12595441	(A, C, and E), although the corresponding membranes  were immunostained with a rabbit anti-GapA polyclonal antibody (B and D) or with  MAb 1E5 that binds the PvpA surface protein (F). "`+"`	bind
52817	2	3448	6	11	NULL	0	NULL	PvpA	GP		is a type of					surface protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_71_3_1265_s_143	12595441	(A, C, and E), although the corresponding membranes  were immunostained with a rabbit anti-GapA polyclonal antibody (B and D) or with  MAb 1E5 that binds the PvpA surface protein (F). "`+"`	bind
10734	1	3448	7	11	NULL	0	NULL	MAb 1E5	GP		bind					PvpA	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_71_3_1265_s_143	12595441	(A, C, and E), although the corresponding membranes  were immunostained with a rabbit anti-GapA polyclonal antibody (B and D) or with  MAb 1E5 that binds the PvpA surface protein (F). "`+"`	bind
52819	2	3448	7	11	NULL	0	NULL	PvpA	GP		is a type of					surface protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_71_3_1265_s_143	12595441	(A, C, and E), although the corresponding membranes  were immunostained with a rabbit anti-GapA polyclonal antibody (B and D) or with  MAb 1E5 that binds the PvpA surface protein (F). "`+"`	bind
80582	1	3448	11	NULL	NULL	0	NULL	MAb 1E5	Protein		binds to 					PvpA	Gene				NULL		0	NULL	NULL	NULL	gw70_infectimmun_71_3_1265_s_143	12595441	(A, C, and E), although the corresponding membranes  were immunostained with a rabbit anti-GapA polyclonal antibody (B and D) or with  MAb 1E5 that binds the PvpA surface protein (F). "`+"`	bind
7700	1	3452	6	11	NULL	0	NULL	amphiphysin	GP		bind					adaptin	GP		appendage domain		NULL	total brain cytosol	NULL	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
7701	2	3452	6	11	NULL	0	NULL	Eps15	GP		bind					adaptin	GP		appendage domain		NULL	total brain cytosol	NULL	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
7702	3	3452	6	11	NULL	0	NULL	AP180	GP		bind					adaptin	GP		appendage domain		NULL	total brain cytosol	NULL	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
7703	4	3452	6	11	NULL	0	NULL	clathrin	GP		bind					adaptin	GP		appendage domain		NULL	total brain cytosol	NULL	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
7704	5	3452	6	11	NULL	0	NULL	DPW peptides	AminoAcid		inhibit					statement 1	Process				NULL	total brain cytosol	NULL	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
7705	6	3452	6	11	NULL	0	NULL	DPW peptides	AminoAcid		inhibits					statement 2	Process				NULL	total brain cytosol	NULL	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
7706	7	3452	6	11	NULL	0	NULL	DPW peptides	AminoAcid		inhibits					statement 3	Process				NULL	total brain cytosol	NULL	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
7707	8	3452	6	11	NULL	0	NULL	DPW peptides	AminoAcid		inhibits					statement 4	Process				NULL	total brain cytosol	NULL	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
7708	9	3452	6	11	NULL	0	NULL	DPF peptides	AminoAcid		inhibits					statement 1	Process				NULL	total brain cytosol	NULL	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
7709	10	3452	6	11	NULL	0	NULL	DPF peptides	AminoAcid		inhibits					statement 2	Process				NULL	total brain cytosol	NULL	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
7710	11	3452	6	11	NULL	0	NULL	DPF peptides	AminoAcid		inhibits					statement 3	Process				NULL	total brain cytosol	NULL	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
7711	12	3452	6	11	NULL	0	NULL	DPF peptides	AminoAcid		inhibits					statement 4	Process				NULL	total brain cytosol	NULL	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
10735	1	3452	7	11	NULL	0	NULL	amphiphysin	GP		bind					adaptin	GP		appendage domain 		NULL	total brain cytosol	NULL	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
10736	2	3452	7	11	NULL	0	NULL	Eps15	GP		bind					adaptin	GP		appendage domain 		NULL	total brain cytosol	NULL	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
10737	3	3452	7	11	NULL	0	NULL	AP180	GP		bind					adaptin	GP		appendage domain 		NULL	total brain cytosol	NULL	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
10738	4	3452	7	11	NULL	0	NULL	clathrin	GP		bind					adaptin	GP		appendage domain 		NULL	total brain cytosol	NULL	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
10739	5	3452	7	11	NULL	0	NULL	DPW peptide	AminoAcid		inhibit					statement 1	Process				NULL	total brain cytosol	NULL	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
10740	6	3452	7	11	NULL	0	NULL	DPW peptide	AminoAcid		inhibit					statement 2	Process				NULL	total brain cytosol	NULL	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
10741	7	3452	7	11	NULL	0	NULL	DPW peptide	AminoAcid		inhibit					statement 3	Process				NULL	total brain cytosol	NULL	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
10742	8	3452	7	11	NULL	0	NULL	DPW peptide	AminoAcid		inhibit					statement 4	Process				NULL	total brain cytosol	NULL	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
10743	9	3452	7	11	NULL	0	NULL	DPF peptide	AminoAcid		inhibit					statement 1	Process				NULL	total brain cytosol	NULL	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
10744	10	3452	7	11	NULL	0	NULL	DPF peptide	AminoAcid		inhibit					statement 2	Process				NULL	total brain cytosol	NULL	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
10745	11	3452	7	11	NULL	0	NULL	DPF peptide	AminoAcid		inhibit					statement 3	Process				NULL	total brain cytosol	NULL	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
10746	12	3452	7	11	NULL	0	NULL	DPF peptide	AminoAcid		inhibit					statement 4	Process				NULL	total brain cytosol	NULL	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
80583	1	3452	11	NULL	NULL	0	NULL	amphiphysin	Protein		binds to 					GST	Protein		adaptin appendage domain		NULL	from total brain cytosol	0	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
80584	2	3452	11	NULL	NULL	0	NULL	Eps15	Protein		binds to 					GST	Protein		adaptin appendage domain		NULL	from total brain cytosol	0	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
80585	3	3452	11	NULL	NULL	0	NULL	AP180	Protein		binds to 					GST	Protein		adaptin appendage domain		NULL	from total brain cytosol	0	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
80586	4	3452	11	NULL	NULL	0	NULL	clathrin	Protein		binds to 					GST	Protein		adaptin appendage domain		NULL	from total brain cytosol	0	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
80587	5	3452	11	NULL	NULL	0	NULL	DPF peptide	PartOfProtein		inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
80588	6	3452	11	NULL	NULL	0	NULL	DPF peptide	PartOfProtein		inhibit					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
80589	7	3452	11	NULL	NULL	0	NULL	DPF peptide	PartOfProtein		inhibit					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
80590	8	3452	11	NULL	NULL	0	NULL	DPW peptide	PartOfProtein		inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
80591	9	3452	11	NULL	NULL	0	NULL	DPW peptide	PartOfProtein		inhibit					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
80592	10	3452	11	NULL	NULL	0	NULL	DPW peptide	PartOfProtein		inhibit					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_cell_97_6_805_s_125	10380931	(A, lower panels), and DPW and DPF  peptides at concentrations of 500 muM (B) inhibit binding of amphiphysin, Eps15, AP180, and clathrin to  GST  -adaptin appendage domain in pull-down experiments from total brain cytosol.	bind
7669	1	3453	6	11	NULL	0	NULL	IGF-I	GP		induce					MC3T3-E1 cells	Cell	chemotaxis of			NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_315_3_636_s_47	14975748	(A,B)  Chemotaxis of MC3T3-E1 cells induced by PDGF, VEGF, and IGF-I.	bind
7670	2	3453	6	11	NULL	0	NULL	VEGF	GP		induce					MC3T3-E1 cells	Cell	chemotaxis of			NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_315_3_636_s_47	14975748	(A,B)  Chemotaxis of MC3T3-E1 cells induced by PDGF, VEGF, and IGF-I.	bind
7671	3	3453	6	11	NULL	0	NULL	PDGF	GP		induce					MC3T3-E1 cells	Cell	chemotaxis of			NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_315_3_636_s_47	14975748	(A,B)  Chemotaxis of MC3T3-E1 cells induced by PDGF, VEGF, and IGF-I.	bind
10747	1	3453	7	11	NULL	0	NULL	PDGF	GP		induce					MC3T3-E1 cells	Cell	chemotaxis of			NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_315_3_636_s_47	14975748	(A,B)  Chemotaxis of MC3T3-E1 cells induced by PDGF, VEGF, and IGF-I.	bind
10748	2	3453	7	11	NULL	0	NULL	VEGF	GP		induce					MC3T3-E1 cells	Cell	chemotaxis of			NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_315_3_636_s_47	14975748	(A,B)  Chemotaxis of MC3T3-E1 cells induced by PDGF, VEGF, and IGF-I.	bind
10749	3	3453	7	11	NULL	0	NULL	IGF-I	GP		induce					MC3T3-E1 cells	Cell	chemotaxis of			NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_315_3_636_s_47	14975748	(A,B)  Chemotaxis of MC3T3-E1 cells induced by PDGF, VEGF, and IGF-I.	bind
80593	1	3453	11	NULL	NULL	0	NULL	PDGF	Protein		induce					Chemotaxis	BiologicalProcess	MC3T3-E1 cells			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_315_3_636_s_47	14975748	(A,B)  Chemotaxis of MC3T3-E1 cells induced by PDGF, VEGF, and IGF-I.	bind
80594	2	3453	11	NULL	NULL	0	NULL	VEGF	Protein		induce					Chemotaxis	BiologicalProcess	MC3T3-E1 cells			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_315_3_636_s_47	14975748	(A,B)  Chemotaxis of MC3T3-E1 cells induced by PDGF, VEGF, and IGF-I.	bind
80596	3	3453	11	NULL	NULL	0	NULL	IGF-I	Protein		induce					Chemotaxis	BiologicalProcess	MC3T3-E1 cells			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_315_3_636_s_47	14975748	(A,B)  Chemotaxis of MC3T3-E1 cells induced by PDGF, VEGF, and IGF-I.	bind
7672	1	3456	6	11	NULL	0	NULL	lectin	GP		bind					gastric mucins	GP	purified;; pig			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1674_2_131_s_139	15374617	(A,B) Lectin binding to purified pig gastric mucins.	bind
10750	1	3456	7	11	NULL	0	NULL	Lectin	GP		bind					gastric mucins	GP	purified;; pig 			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1674_2_131_s_139	15374617	(A,B) Lectin binding to purified pig gastric mucins.	bind
80602	1	3456	11	NULL	NULL	0	NULL	Lectin	Protein		binds to 					gastric mucin	Chemical	purified;;pig			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1674_2_131_s_139	15374617	(A,B) Lectin binding to purified pig gastric mucins.	bind
7673	1	3459	6	11	NULL	0	NULL	SPRY2	GP		bind					GRB2	GP				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_96_1_91_s_85	10940627	(A,B) SPRY2 binds GRB2.	bind
10818	1	3459	7	11	NULL	0	NULL	SPRY2	GP		bind					GRB2	GP				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_96_1_91_s_85	10940627	(A,B) SPRY2 binds GRB2.	bind
80603	1	3459	11	NULL	NULL	0	NULL	SPRY2	Protein		binds to 					GRB2	Protein				NULL		0	NULL	NULL	NULL	gw60_mechdev_96_1_91_s_85	10940627	(A,B) SPRY2 binds GRB2.	bind
7719	1	3460	6	11	NULL	0	NULL	prazosin	Chemical		bind			BODIPY FL		alpha-1 adrenoceptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_132_4_851_s_194	11181426	(A,B) the cells were incubated in the presence of BODIPY FL prazosin and unlabelled prazosin 10-6M (which blocks the binding of BODIPY FL prazosin to the alpha-1 adrenoceptors).	bind
7720	2	3460	6	11	NULL	0	NULL	prazosin	Chemical	unlabelled	blocks					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_132_4_851_s_194	11181426	(A,B) the cells were incubated in the presence of BODIPY FL prazosin and unlabelled prazosin 10-6M (which blocks the binding of BODIPY FL prazosin to the alpha-1 adrenoceptors).	bind
10819	1	3460	7	11	NULL	0	NULL	 prazosin	Chemical		bind			BODIPY FL		alpha-1 adrenoceptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_132_4_851_s_194	11181426	(A,B) the cells were incubated in the presence of BODIPY FL prazosin and unlabelled prazosin 10-6M (which blocks the binding of BODIPY FL prazosin to the alpha-1 adrenoceptors).	bind
14982	2	3460	7	11	NULL	0	NULL	prazosin	Chemical	unlabelled 	blocks					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_132_4_851_s_194	11181426	(A,B) the cells were incubated in the presence of BODIPY FL prazosin and unlabelled prazosin 10-6M (which blocks the binding of BODIPY FL prazosin to the alpha-1 adrenoceptors).	bind
80604	1	3460	11	NULL	NULL	0	NULL	BODIPY FL prazosin	Chemical		binds to 					alpha-1 adrenoceptors	Protein				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_132_4_851_s_194	11181426	(A,B) the cells were incubated in the presence of BODIPY FL prazosin and unlabelled prazosin 10-6M (which blocks the binding of BODIPY FL prazosin to the alpha-1 adrenoceptors).	bind
80605	2	3460	11	NULL	NULL	0	NULL	prazosin	Chemical	unlabelled	blocks					statement 1	Chemical				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_132_4_851_s_194	11181426	(A,B) the cells were incubated in the presence of BODIPY FL prazosin and unlabelled prazosin 10-6M (which blocks the binding of BODIPY FL prazosin to the alpha-1 adrenoceptors).	bind
7674	1	3461	6	11	NULL	0	NULL	GPA-16	GP		bind					GST-GPR-1/2	GP		amino acids 374-476		NULL		NULL	NULL	NULL	NULL	gw70_development_132_20_4449_s_203	16162648	(A,B,E) [[ Surface plasmon  resonance ]] was used to analyze the binding of GPA-16 to GST-GPR-1/2 (amino acids 374-476)	bind
10820	1	3461	7	11	NULL	0	NULL	GPA-16	GP		bind					GST-GPR-1/2 	GP		374-476		NULL		NULL	NULL	NULL	NULL	gw70_development_132_20_4449_s_203	16162648	(A,B,E) [[ Surface plasmon  resonance ]] was used to analyze the binding of GPA-16 to GST-GPR-1/2 (amino acids 374-476)	bind
80606	1	3461	11	NULL	NULL	0	NULL	GPA-16	Protein		binds to 					GST-GPR-1/2	Protein		amino acids 374-476		NULL		0	NULL	NULL	NULL	gw70_development_132_20_4449_s_203	16162648	(A,B,E) [[ Surface plasmon  resonance ]] was used to analyze the binding of GPA-16 to GST-GPR-1/2 (amino acids 374-476)	bind
7721	1	3463	6	11	NULL	0	NULL	D-type cyclins	GP		bind					CDK4	GP		cyclin binding sequence		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7041_s_19	11096103	(A- and B-type) bind CDKs that contain the conserved cyclin-binding sequence PSTAIRE, whereas D-type cyclins bind CDK4 and -6, which have the sequence P(I/L)ST(V/I)RE (reviewed in Ref.  13).	bind
7722	2	3463	6	11	NULL	0	NULL	D-type cyclins	GP		bind					CDK6	GP		cyclin binding sequence		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7041_s_19	11096103	(A- and B-type) bind CDKs that contain the conserved cyclin-binding sequence PSTAIRE, whereas D-type cyclins bind CDK4 and -6, which have the sequence P(I/L)ST(V/I)RE (reviewed in Ref.  13).	bind
7751	3	3463	6	11	NULL	0	NULL	P(I/L)ST(V/I)RE	NucleicAcid		is a type of					cyclin binding sequence	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7041_s_19	11096103	(A- and B-type) bind CDKs that contain the conserved cyclin-binding sequence PSTAIRE, whereas D-type cyclins bind CDK4 and -6, which have the sequence P(I/L)ST(V/I)RE (reviewed in Ref.  13).	bind
10823	3	3463	7	11	NULL	0	NULL	D-type cyclins	GP		bind					CDK4	GP		P(I/L)ST(V/I)RE		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7041_s_19	11096103	(A- and B-type) bind CDKs that contain the conserved cyclin-binding sequence PSTAIRE, whereas D-type cyclins bind CDK4 and -6, which have the sequence P(I/L)ST(V/I)RE (reviewed in Ref.  13).	bind
10824	4	3463	7	11	NULL	0	NULL	D-type cyclins	GP		bind					CDK6	GP		P(I/L)ST(V/I)RE		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7041_s_19	11096103	(A- and B-type) bind CDKs that contain the conserved cyclin-binding sequence PSTAIRE, whereas D-type cyclins bind CDK4 and -6, which have the sequence P(I/L)ST(V/I)RE (reviewed in Ref.  13).	bind
52826	5	3463	7	11	NULL	0	NULL	P(I/L)ST(V/I)RE	NucleicAcid		is a type of					cyclin binding sequence	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7041_s_19	11096103	(A- and B-type) bind CDKs that contain the conserved cyclin-binding sequence PSTAIRE, whereas D-type cyclins bind CDK4 and -6, which have the sequence P(I/L)ST(V/I)RE (reviewed in Ref.  13).	bind
80607	1	3463	11	NULL	NULL	0	NULL	PSTAIRE	PartOfProtein		is a part of 					cyclin-binding sequence	PartOfProtein	conserved			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_10_7041_s_19	11096103	(A- and B-type) bind CDKs that contain the conserved cyclin-binding sequence PSTAIRE, whereas D-type cyclins bind CDK4 and -6, which have the sequence P(I/L)ST(V/I)RE (reviewed in Ref.  13).	bind
80608	2	3463	11	NULL	NULL	0	NULL	CDK	Protein		contain					PSTAIRE	PartOfProtein				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_10_7041_s_19	11096103	(A- and B-type) bind CDKs that contain the conserved cyclin-binding sequence PSTAIRE, whereas D-type cyclins bind CDK4 and -6, which have the sequence P(I/L)ST(V/I)RE (reviewed in Ref.  13).	bind
80609	3	3463	11	NULL	NULL	NULL	NULL	D-type cyclin	Protein		binds to 					CDK4	Protein		P(I/L)ST(V/I)RE		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7041_s_19	11096103	(A- and B-type) bind CDKs that contain the conserved cyclin-binding sequence PSTAIRE, whereas D-type cyclins bind CDK4 and -6, which have the sequence P(I/L)ST(V/I)RE (reviewed in Ref.  13).	bind
80610	4	3463	11	NULL	NULL	NULL	NULL	D-type cyclin	Protein		binds to 					CDK6	Protein		P(I/L)ST(V/I)RE		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7041_s_19	11096103	(A- and B-type) bind CDKs that contain the conserved cyclin-binding sequence PSTAIRE, whereas D-type cyclins bind CDK4 and -6, which have the sequence P(I/L)ST(V/I)RE (reviewed in Ref.  13).	bind
7677	1	3464	6	11	NULL	0	NULL	Sir1p	GP		bind					HMR a	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_5_1955_s_197	16479013	(A-) still requires  SIR1 (Palacios DeBeer and Fox, unpublished), indicating that Sir1p must bind  HMR a in this mutant by some mechanism.	bind
10825	1	3464	7	11	NULL	0	NULL	Sir1p 	GP		bind					HMR a	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_5_1955_s_197	16479013	(A-) still requires  SIR1 (Palacios DeBeer and Fox, unpublished), indicating that Sir1p must bind  HMR a in this mutant by some mechanism.	bind
80611	1	3464	11	NULL	NULL	0	NULL	Sir1p	Protein		binds to 					HMRa	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_5_1955_s_197	16479013	(A-) still requires  SIR1 (Palacios DeBeer and Fox, unpublished), indicating that Sir1p must bind  HMR a in this mutant by some mechanism.	bind
7723	1	3465	6	11	NULL	0	NULL	 IL-3 	GP	murine	bind		directly			beta(IL-3)receptor	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_j-biol-chem_279_25_15060062_s_9	15060062	(A-B loop), Phe(85), and Asn(87) (E-F loop) of  domain 1; Ile(320) of the interdomain loop; and Tyr(348) (B''-C'' loop)  and Tyr(401) (F''-G'' loop) of domain 4 were shown to have critical individual  roles and Arg(84) and Tyr(317) major secondary roles in direct murine  IL-3 binding to the beta(IL-3)receptor.	bind
7752	2	3465	6	11	NULL	0	NULL				plays critical role in			Phe(85);;Asn(87) (E-F loop) of domain 1		statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_j-biol-chem_279_25_15060062_s_9	15060062	(A-B loop), Phe(85), and Asn(87) (E-F loop) of  domain 1; Ile(320) of the interdomain loop; and Tyr(348) (B''-C'' loop)  and Tyr(401) (F''-G'' loop) of domain 4 were shown to have critical individual  roles and Arg(84) and Tyr(317) major secondary roles in direct murine  IL-3 binding to the beta(IL-3)receptor.	bind
7753	3	3465	6	11	NULL	0	NULL				plays critical role in			Ile(320) of the interdomain loop		statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_j-biol-chem_279_25_15060062_s_9	15060062	(A-B loop), Phe(85), and Asn(87) (E-F loop) of  domain 1; Ile(320) of the interdomain loop; and Tyr(348) (B''-C'' loop)  and Tyr(401) (F''-G'' loop) of domain 4 were shown to have critical individual  roles and Arg(84) and Tyr(317) major secondary roles in direct murine  IL-3 binding to the beta(IL-3)receptor.	bind
7754	4	3465	6	11	NULL	0	NULL				plays critical role in			Tyr(348) (B''-C'' loop)		statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_j-biol-chem_279_25_15060062_s_9	15060062	(A-B loop), Phe(85), and Asn(87) (E-F loop) of  domain 1; Ile(320) of the interdomain loop; and Tyr(348) (B''-C'' loop)  and Tyr(401) (F''-G'' loop) of domain 4 were shown to have critical individual  roles and Arg(84) and Tyr(317) major secondary roles in direct murine  IL-3 binding to the beta(IL-3)receptor.	bind
7755	5	3465	6	11	NULL	0	NULL				plays critical role in			Tyr(401) (F''-G'' loop) of domain 4		statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_j-biol-chem_279_25_15060062_s_9	15060062	(A-B loop), Phe(85), and Asn(87) (E-F loop) of  domain 1; Ile(320) of the interdomain loop; and Tyr(348) (B''-C'' loop)  and Tyr(401) (F''-G'' loop) of domain 4 were shown to have critical individual  roles and Arg(84) and Tyr(317) major secondary roles in direct murine  IL-3 binding to the beta(IL-3)receptor.	bind
7756	6	3465	6	11	NULL	0	NULL	Arg(84)			plays major secondary role in					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_j-biol-chem_279_25_15060062_s_9	15060062	(A-B loop), Phe(85), and Asn(87) (E-F loop) of  domain 1; Ile(320) of the interdomain loop; and Tyr(348) (B''-C'' loop)  and Tyr(401) (F''-G'' loop) of domain 4 were shown to have critical individual  roles and Arg(84) and Tyr(317) major secondary roles in direct murine  IL-3 binding to the beta(IL-3)receptor.	bind
7757	7	3465	6	11	NULL	0	NULL	Tyr(317)	AminoAcid		plays major secondary role in					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_j-biol-chem_279_25_15060062_s_9	15060062	(A-B loop), Phe(85), and Asn(87) (E-F loop) of  domain 1; Ile(320) of the interdomain loop; and Tyr(348) (B''-C'' loop)  and Tyr(401) (F''-G'' loop) of domain 4 were shown to have critical individual  roles and Arg(84) and Tyr(317) major secondary roles in direct murine  IL-3 binding to the beta(IL-3)receptor.	bind
10826	1	3465	7	11	NULL	0	NULL	IL-3	GP	murine	bind		directly			beta(IL-3)receptor	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_j-biol-chem_279_25_15060062_s_9	15060062	(A-B loop), Phe(85), and Asn(87) (E-F loop) of  domain 1; Ile(320) of the interdomain loop; and Tyr(348) (B''-C'' loop)  and Tyr(401) (F''-G'' loop) of domain 4 were shown to have critical individual  roles and Arg(84) and Tyr(317) major secondary roles in direct murine  IL-3 binding to the beta(IL-3)receptor.	bind
10827	2	3465	7	11	NULL	0	NULL				has critical role in			Phe(85);;Asn(87) (E-F loop) of domain 1		statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_j-biol-chem_279_25_15060062_s_9	15060062	(A-B loop), Phe(85), and Asn(87) (E-F loop) of  domain 1; Ile(320) of the interdomain loop; and Tyr(348) (B''-C'' loop)  and Tyr(401) (F''-G'' loop) of domain 4 were shown to have critical individual  roles and Arg(84) and Tyr(317) major secondary roles in direct murine  IL-3 binding to the beta(IL-3)receptor.	bind
10829	4	3465	7	11	NULL	0	NULL				has critical role in			Ile(320) of the interdomain loop		statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_j-biol-chem_279_25_15060062_s_9	15060062	(A-B loop), Phe(85), and Asn(87) (E-F loop) of  domain 1; Ile(320) of the interdomain loop; and Tyr(348) (B''-C'' loop)  and Tyr(401) (F''-G'' loop) of domain 4 were shown to have critical individual  roles and Arg(84) and Tyr(317) major secondary roles in direct murine  IL-3 binding to the beta(IL-3)receptor.	bind
10830	5	3465	7	11	NULL	0	NULL				has critical role in			Tyr(348) (B''-C'' loop) of domain 4		statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_j-biol-chem_279_25_15060062_s_9	15060062	(A-B loop), Phe(85), and Asn(87) (E-F loop) of  domain 1; Ile(320) of the interdomain loop; and Tyr(348) (B''-C'' loop)  and Tyr(401) (F''-G'' loop) of domain 4 were shown to have critical individual  roles and Arg(84) and Tyr(317) major secondary roles in direct murine  IL-3 binding to the beta(IL-3)receptor.	bind
10831	6	3465	7	11	NULL	0	NULL				has critical role in			Tyr(401) (F''-G'' loop) of domain 4		statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_j-biol-chem_279_25_15060062_s_9	15060062	(A-B loop), Phe(85), and Asn(87) (E-F loop) of  domain 1; Ile(320) of the interdomain loop; and Tyr(348) (B''-C'' loop)  and Tyr(401) (F''-G'' loop) of domain 4 were shown to have critical individual  roles and Arg(84) and Tyr(317) major secondary roles in direct murine  IL-3 binding to the beta(IL-3)receptor.	bind
10832	7	3465	7	11	NULL	0	NULL	Arg(84)	AminoAcid		has major secondary role in					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_j-biol-chem_279_25_15060062_s_9	15060062	(A-B loop), Phe(85), and Asn(87) (E-F loop) of  domain 1; Ile(320) of the interdomain loop; and Tyr(348) (B''-C'' loop)  and Tyr(401) (F''-G'' loop) of domain 4 were shown to have critical individual  roles and Arg(84) and Tyr(317) major secondary roles in direct murine  IL-3 binding to the beta(IL-3)receptor.	bind
10833	8	3465	7	11	NULL	0	NULL	Tyr(317)	AminoAcid		has major secondary role in					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_j-biol-chem_279_25_15060062_s_9	15060062	(A-B loop), Phe(85), and Asn(87) (E-F loop) of  domain 1; Ile(320) of the interdomain loop; and Tyr(348) (B''-C'' loop)  and Tyr(401) (F''-G'' loop) of domain 4 were shown to have critical individual  roles and Arg(84) and Tyr(317) major secondary roles in direct murine  IL-3 binding to the beta(IL-3)receptor.	bind
80612	1	3465	11	NULL	NULL	0	NULL	IL-3	Protein	murine	binds to 		direct			beta(IL-3)receptor	Protein				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-biol-chem_279_25_15060062_s_9	15060062	(A-B loop), Phe(85), and Asn(87) (E-F loop) of  domain 1; Ile(320) of the interdomain loop; and Tyr(348) (B''-C'' loop)  and Tyr(401) (F''-G'' loop) of domain 4 were shown to have critical individual  roles and Arg(84) and Tyr(317) major secondary roles in direct murine  IL-3 binding to the beta(IL-3)receptor.	bind
7681	1	3466	6	11	NULL	0	NULL	3H-CGP 39653	Chemical		bind					spinal cord sections	OrganismPart	mouse			NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_86_1_23_s_117	11165368	(A-B) Autoradiograms showing binding of 3H-CGP 39653 to sections of mouse spinal cord.	bind
10834	1	3466	7	11	NULL	0	NULL	3H-CGP 39653	Chemical		bind					 spinal cord	OrganismPart	mouse			NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_86_1_23_s_117	11165368	(A-B) Autoradiograms showing binding of 3H-CGP 39653 to sections of mouse spinal cord.	bind
80625	1	3466	11	NULL	NULL	0	NULL	3H-CGP 39653	PartOfProtein		binds to 					spinal cord	Organism part	mouse			NULL		0	NULL	NULL	NULL	gw60_brainresmolbrainres_86_1_23_s_117	11165368	(A-B) Autoradiograms showing binding of 3H-CGP 39653 to sections of mouse spinal cord.	bind
7682	1	3467	6	11	NULL	0	NULL	Bcr	GP		does not bind					Max	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_13_5_437_s_106	12620195	(A-C) Bcr does not bind Max or the c-Myc Max heterodimer.	bind
7683	2	3467	6	11	NULL	0	NULL	Bcr	GP		does not bind					c-Myc Max heterodimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_13_5_437_s_106	12620195	(A-C) Bcr does not bind Max or the c-Myc Max heterodimer.	bind
10835	1	3467	7	11	NULL	0	NULL	Bcr 	GP		does not bind					 Max	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_13_5_437_s_106	12620195	(A-C) Bcr does not bind Max or the c-Myc Max heterodimer.	bind
10836	2	3467	7	11	NULL	0	NULL	Bcr	GP		does not bind					c-Myc Max heterodimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_13_5_437_s_106	12620195	(A-C) Bcr does not bind Max or the c-Myc Max heterodimer.	bind
80627	1	3467	11	NULL	NULL	0	NULL	 c-Myc	Protein		heterodimerize with					Max	Protein				NULL		0	NULL	NULL	NULL	gw60_currbiol_13_5_437_s_106	12620195	(A-C) Bcr does not bind Max or the c-Myc Max heterodimer.	bind
80629	2	3467	11	NULL	NULL	0	NULL	Bcr	Protein		does not bind to					Max	Protein				NULL		0	NULL	NULL	NULL	gw60_currbiol_13_5_437_s_106	12620195	(A-C) Bcr does not bind Max or the c-Myc Max heterodimer.	bind
80630	3	3467	11	NULL	NULL	0	NULL	Bcr	Protein		does not bind to					statement 1	Protein				NULL		0	NULL	NULL	NULL	gw60_currbiol_13_5_437_s_106	12620195	(A-C) Bcr does not bind Max or the c-Myc Max heterodimer.	bind
7724	1	3468	6	11	NULL	0	NULL	RF3 GDPNP	GP		bind					RC	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
7725	2	3468	6	11	NULL	0	NULL	RF3 GDPNP	GP		bind					IC	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
7726	3	3468	6	11	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
7727	4	3468	6	11	NULL	0	NULL	statement 1	Process		occurs in presence of					deacylated tRNA in the P site	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
7728	5	3468	6	11	NULL	0	NULL	statement 1	Process		occurs in presence of					peptidyl-tRNA in the P site	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
7729	6	3468	6	11	NULL	0	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
7730	7	3468	6	11	NULL	0	NULL	statement 2	Process		occurs in presence of					deacylated tRNA in the P site	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
7731	8	3468	6	11	NULL	0	NULL	statement 2	Process		occurs in presence of					peptidyl-tRNA in the P site	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
7732	9	3468	6	11	NULL	0	NULL	statement 7	Process		is an alternative to					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
7758	10	3468	6	11	NULL	0	NULL	EF-G GDPNP	GP		bind					RC	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
7759	11	3468	6	11	NULL	0	NULL	EF-G GDPNP	GP		bind					IC	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
7760	12	3468	6	11	NULL	0	NULL	statement 10	Process		is an alternative to					statement 11	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
7763	13	3468	6	11	NULL	0	NULL	statement 10	Process		occurs in presence of					deacylated tRNA in the P site	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
7764	14	3468	6	11	NULL	0	NULL	statement 10	Process		occurs in presence of					peptidyl-tRNA in the P site	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
7765	15	3468	6	11	NULL	0	NULL	statement 13	Process		is an alternative to					statement 14	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
7766	16	3468	6	11	NULL	0	NULL	statement 11	Process		occurs in presence of					peptidyl-tRNA in the P site	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
7767	17	3468	6	11	NULL	0	NULL	statement 11	Process		occurs in presence of					deacetylated-tRNA in the P site	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
7769	18	3468	6	11	NULL	0	NULL	statement 16	Process		is an alternative to					statement 17	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
7770	19	3468	6	11	NULL	0	NULL	IF2 GDPNP	GP		bind					RC	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
7771	20	3468	6	11	NULL	0	NULL	IF2 GDPNP	GP		bind					IC	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
7776	21	3468	6	11	NULL	0	NULL	statement 19	Process		is an alternative to					statement 20	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
7778	22	3468	6	11	NULL	0	NULL	statement 19	Process		occurs in presence of					deacetylated-tRNA in the P site	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
7779	23	3468	6	11	NULL	0	NULL	statement 19	Process		occurs in presence of					peptidyl-tRNA in the P site	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
7781	24	3468	6	11	NULL	0	NULL	statement 22	Process		is an alternative to					statement 23	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
7782	25	3468	6	11	NULL	0	NULL	statement 20	Process		occurs in presence of					peptidyl-tRNA in the P site	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
7783	26	3468	6	11	NULL	0	NULL	statement 20	Process		occurs in presence of					deacetylated-tRNA in the P site	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
7785	27	3468	6	11	NULL	0	NULL	statement 25	Process		is an alternative to					statement 26	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
10844	1	3468	7	11	NULL	0	NULL	RF3 GDPNP	GP		bind					IC	GP			peptidyl-tRNA in the P site 	NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
10845	2	3468	7	11	NULL	0	NULL	RF3 GDPNP	GP		bind					RC	GP			deacylated tRNA in the P site	NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
10846	3	3468	7	11	NULL	0	NULL	RF3 GDPNP	GP		bind					IC	GP			deacylated tRNA in the P site	NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
10847	5	3468	7	11	NULL	0	NULL	EF-G GDPNP	GP		bind					RC	GP			peptidyl-tRNA in the P site 	NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
10848	4	3468	7	11	NULL	0	NULL	 RF3 GDPNP	GP		bind					RC	GP			peptidyl-tRNA in the P site 	NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
10849	7	3468	7	11	NULL	0	NULL	EF-G GDPNP	GP		bind					IC	GP			peptidyl-tRNA in the P site 	NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
10850	8	3468	7	11	NULL	0	NULL	EF-G GDPNP	GP		bind					IC	GP			deacylated tRNA in the P site	NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
10851	9	3468	7	11	NULL	0	NULL	IF2 GDPNP	GP		bind					RC	GP			peptidyl-tRNA in the P site 	NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
10852	10	3468	7	11	NULL	0	NULL	IF2 GDPNP	GP		bind					RC	GP			deacylated tRNA in the P site	NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
10853	11	3468	7	11	NULL	0	NULL	IF2 GDPNP	GP		bind					IC	GP			peptidyl-tRNA in the P site 	NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
10854	6	3468	7	11	NULL	0	NULL	EF-G GDPNP	GP		bind					RC	GP			deacylated tRNA in the P site	NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
10855	12	3468	7	11	NULL	0	NULL	IF2 GDPNP	GP		bind					IC	GP			deacylated tRNA in the P site	NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
80631	1	3468	11	NULL	NULL	NULL	NULL	RF3 GDPNP	Protein		binds to 					RC	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
80632	2	3468	11	NULL	NULL	NULL	NULL	EF-G GDPNP	Protein		binds to 					RC	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
80633	3	3468	11	NULL	NULL	NULL	NULL	IF2 GDPNP	Protein		binds to 					RC	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
80634	4	3468	11	NULL	NULL	0	NULL	RC	CellComponent		has					 peptidyl-tRNA	CellComponent	in the P site			NULL		0	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
80635	5	3468	11	NULL	NULL	0	NULL	RC	CellComponent		has					deacylated tRNA	CellComponent	in the P site			NULL		0	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
80636	6	3468	11	NULL	NULL	0	NULL	 IC	Protein		with					peptidyl-tRNA	CellComponent	in the P site			NULL		0	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
80637	7	3468	11	NULL	NULL	0	NULL	IC	Protein		with					deacylated tRNA	CellComponent	in the P site			NULL		0	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
80650	8	3468	11	NULL	NULL	0	NULL	RF3 GDPNP	Protein		binds to 					IC	Protein				NULL		0	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
80662	9	3468	11	NULL	NULL	0	NULL	EF-G GDPNP	Protein		binds to 					IC	Protein				NULL		0	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
80664	10	3468	11	NULL	NULL	0	NULL	IF2 GDPNP	Protein		binds to 					IC	Protein				NULL		0	NULL	NULL	NULL	gw60_cell_114_1_113_s_67	12859902	(A-C) Binding of RF3 GDPNP, EF-G GDPNP, and IF2 GDPNP to RC or IC with peptidyl-tRNA or deacylated tRNA in the P site.	bind
7685	1	3469	6	11	NULL	0	NULL	dATP	Chemical		bind					RVLM	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_113_4_809_s_145	12182888	(A-C) Binding of [ 33]dATP can be seen in a number of brainstem regions, including the RVLM, CVLM and IOC.	bind
7686	2	3469	6	11	NULL	0	NULL	dATP	Chemical		bind					CVLM	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_113_4_809_s_145	12182888	(A-C) Binding of [ 33]dATP can be seen in a number of brainstem regions, including the RVLM, CVLM and IOC.	bind
7687	3	3469	6	11	NULL	0	NULL	dATP	Chemical		bind					IOC	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_113_4_809_s_145	12182888	(A-C) Binding of [ 33]dATP can be seen in a number of brainstem regions, including the RVLM, CVLM and IOC.	bind
52843	4	3469	6	11	NULL	0	NULL	RVLM	OrganismPart		is a type of					brainstem region	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_113_4_809_s_145	12182888	(A-C) Binding of [ 33]dATP can be seen in a number of brainstem regions, including the RVLM, CVLM and IOC.	bind
52844	5	3469	6	11	NULL	0	NULL	CVLM 	OrganismPart		is a type of					brainstem region	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_113_4_809_s_145	12182888	(A-C) Binding of [ 33]dATP can be seen in a number of brainstem regions, including the RVLM, CVLM and IOC.	bind
52845	6	3469	6	11	NULL	0	NULL	IOC	OrganismPart		is a type of					brainstem region	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_113_4_809_s_145	12182888	(A-C) Binding of [ 33]dATP can be seen in a number of brainstem regions, including the RVLM, CVLM and IOC.	bind
10856	1	3469	7	11	NULL	0	NULL	dATP	Chemical		bind					RVLM	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_113_4_809_s_145	12182888	(A-C) Binding of [ 33]dATP can be seen in a number of brainstem regions, including the RVLM, CVLM and IOC.	bind
10857	2	3469	7	11	NULL	0	NULL	dATP	Chemical		bind					CVLM	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_113_4_809_s_145	12182888	(A-C) Binding of [ 33]dATP can be seen in a number of brainstem regions, including the RVLM, CVLM and IOC.	bind
10858	3	3469	7	11	NULL	0	NULL	dATP	Chemical		bind					IOC	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_113_4_809_s_145	12182888	(A-C) Binding of [ 33]dATP can be seen in a number of brainstem regions, including the RVLM, CVLM and IOC.	bind
52846	4	3469	7	11	NULL	0	NULL	RVLM	OrganismPart		is a type of					brainstem region	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_113_4_809_s_145	12182888	(A-C) Binding of [ 33]dATP can be seen in a number of brainstem regions, including the RVLM, CVLM and IOC.	bind
52847	5	3469	7	11	NULL	0	NULL	CVLM 	OrganismPart		is a type of					brainstem region	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_113_4_809_s_145	12182888	(A-C) Binding of [ 33]dATP can be seen in a number of brainstem regions, including the RVLM, CVLM and IOC.	bind
52848	6	3469	7	11	NULL	0	NULL	IOC	OrganismPart		is a type of					brainstem region	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_113_4_809_s_145	12182888	(A-C) Binding of [ 33]dATP can be seen in a number of brainstem regions, including the RVLM, CVLM and IOC.	bind
80666	1	3469	11	NULL	NULL	0	NULL	[ 33]dATP	Chemical		binds to 		(A-C)			RVLM	AnatomicalPart	brainstem region			NULL		0	NULL	NULL	NULL	gw60_neuroscience_113_4_809_s_145	12182888	(A-C) Binding of [ 33]dATP can be seen in a number of brainstem regions, including the RVLM, CVLM and IOC.	bind
80667	2	3469	11	NULL	NULL	0	NULL	 [ 33]dATP	Chemical		binds to 		A-C			CVLM	AnatomicalPart	brainstem region			NULL		0	NULL	NULL	NULL	gw60_neuroscience_113_4_809_s_145	12182888	(A-C) Binding of [ 33]dATP can be seen in a number of brainstem regions, including the RVLM, CVLM and IOC.	bind
80668	3	3469	11	NULL	NULL	0	NULL	[ 33]dATP	Chemical		binds to 		(A-C)			IOC	AnatomicalPart	brainstem region			NULL		0	NULL	NULL	NULL	gw60_neuroscience_113_4_809_s_145	12182888	(A-C) Binding of [ 33]dATP can be seen in a number of brainstem regions, including the RVLM, CVLM and IOC.	bind
7688	1	3470	6	11	NULL	0	NULL	 roX1 RNA	NucleicAcid		bind					polytene X chromosome	Chromosome				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_3_136_s_63	10679323	(a-c) RNA fluorescence  in situ hybridization showing the polytene X chromosome binding pattern of (a)  roX1 RNA and (b)  roX2 RNA.	bind
7689	2	3470	6	11	NULL	0	NULL	 roX2 RNA	NucleicAcid		bind					polytene X chromosome	Chromosome				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_3_136_s_63	10679323	(a-c) RNA fluorescence  in situ hybridization showing the polytene X chromosome binding pattern of (a)  roX1 RNA and (b)  roX2 RNA.	bind
10859	1	3470	7	11	NULL	0	NULL	polytene X chromosome	Chromosome		bind					roX1 RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_3_136_s_63	10679323	(a-c) RNA fluorescence  in situ hybridization showing the polytene X chromosome binding pattern of (a)  roX1 RNA and (b)  roX2 RNA.	bind
10860	2	3470	7	11	NULL	0	NULL	polytene X chromosome	Chromosome		bind					roX2 RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_3_136_s_63	10679323	(a-c) RNA fluorescence  in situ hybridization showing the polytene X chromosome binding pattern of (a)  roX1 RNA and (b)  roX2 RNA.	bind
80671	1	3470	11	NULL	NULL	0	NULL	roX1 RNA	NucleicAcidSubstance		binds to 					 polytene X chromosome	Chromosome				NULL	RNA fluorescence in situ hybridization	0	NULL	NULL	NULL	gw60_currbiol_10_3_136_s_63	10679323	(a-c) RNA fluorescence  in situ hybridization showing the polytene X chromosome binding pattern of (a)  roX1 RNA and (b)  roX2 RNA.	bind
80674	2	3470	11	NULL	NULL	0	NULL	roX2 RNA	NucleicAcidSubstance		binds to 					polytene X chromosome	Chromosome				NULL	RNA fluorescence in situ hybridization	0	NULL	NULL	NULL	gw60_currbiol_10_3_136_s_63	10679323	(a-c) RNA fluorescence  in situ hybridization showing the polytene X chromosome binding pattern of (a)  roX1 RNA and (b)  roX2 RNA.	bind
7690	1	3471	6	11	NULL	0	NULL	HNf-4	GP		bind					Smad3	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_3_1279_s_250	12631740	(A-C) Two regions of HNF-4 defined by amino acids 1-49 (domain A/B) and 388-455 (domain  F) mediate binding of HNF-4 to Smad3.	bind
7691	2	3471	6	11	NULL	0	NULL	HNF-4	GP		mediates			domain A/B		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_3_1279_s_250	12631740	(A-C) Two regions of HNF-4 defined by amino acids 1-49 (domain A/B) and 388-455 (domain  F) mediate binding of HNF-4 to Smad3.	bind
7692	3	3471	6	11	NULL	0	NULL	HNF-4	GP		mediates			domain F		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_3_1279_s_250	12631740	(A-C) Two regions of HNF-4 defined by amino acids 1-49 (domain A/B) and 388-455 (domain  F) mediate binding of HNF-4 to Smad3.	bind
7693	4	3471	6	11	NULL	0	NULL	HNF-4	GP		corresponds to			amino acids 1-49		HNF-4	GP		domain A/B		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_3_1279_s_250	12631740	(A-C) Two regions of HNF-4 defined by amino acids 1-49 (domain A/B) and 388-455 (domain  F) mediate binding of HNF-4 to Smad3.	bind
7694	5	3471	6	11	NULL	0	NULL	HNF-4	GP		corresponds to			amino acids 388-455		HNF-4	GP		domain F		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_3_1279_s_250	12631740	(A-C) Two regions of HNF-4 defined by amino acids 1-49 (domain A/B) and 388-455 (domain  F) mediate binding of HNF-4 to Smad3.	bind
10861	1	3471	7	11	NULL	0	NULL	HNF-4	GP		corresponds to			domain A/B		HNF-4	GP		amino acids 1-49		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_3_1279_s_250	12631740	(A-C) Two regions of HNF-4 defined by amino acids 1-49 (domain A/B) and 388-455 (domain  F) mediate binding of HNF-4 to Smad3.	bind
10862	2	3471	7	11	NULL	0	NULL	HNF-4	GP		corresponds to			 domain F		HNF-4	GP		amino acids 388-455		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_3_1279_s_250	12631740	(A-C) Two regions of HNF-4 defined by amino acids 1-49 (domain A/B) and 388-455 (domain  F) mediate binding of HNF-4 to Smad3.	bind
14994	3	3471	7	11	NULL	0	NULL	HNF-4	GP		bind					Smad3	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_3_1279_s_250	12631740	(A-C) Two regions of HNF-4 defined by amino acids 1-49 (domain A/B) and 388-455 (domain  F) mediate binding of HNF-4 to Smad3.	bind
14995	4	3471	7	11	NULL	0	NULL	statement 1	Process		mediate					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_3_1279_s_250	12631740	(A-C) Two regions of HNF-4 defined by amino acids 1-49 (domain A/B) and 388-455 (domain  F) mediate binding of HNF-4 to Smad3.	bind
14996	5	3471	7	11	NULL	0	NULL	statement 2	Process		mediate					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_3_1279_s_250	12631740	(A-C) Two regions of HNF-4 defined by amino acids 1-49 (domain A/B) and 388-455 (domain  F) mediate binding of HNF-4 to Smad3.	bind
80675	1	3471	11	NULL	NULL	0	NULL	HNF-4 	Protein		binds to 					Smad3	Protein				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_3_1279_s_250	12631740	(A-C) Two regions of HNF-4 defined by amino acids 1-49 (domain A/B) and 388-455 (domain  F) mediate binding of HNF-4 to Smad3.	bind
80677	2	3471	11	NULL	NULL	NULL	NULL				is a part of 			domain A/B;;amino acids 1-49		HNF-4	Protein				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_3_1279_s_250	12631740	(A-C) Two regions of HNF-4 defined by amino acids 1-49 (domain A/B) and 388-455 (domain  F) mediate binding of HNF-4 to Smad3.	bind
80678	3	3471	11	NULL	NULL	0	NULL				is a part of 			domain F;;388-455		HNF-4 	Protein				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_3_1279_s_250	12631740	(A-C) Two regions of HNF-4 defined by amino acids 1-49 (domain A/B) and 388-455 (domain  F) mediate binding of HNF-4 to Smad3.	bind
80681	4	3471	11	NULL	NULL	0	NULL	statement 2	Protein		mediates					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_3_1279_s_250	12631740	(A-C) Two regions of HNF-4 defined by amino acids 1-49 (domain A/B) and 388-455 (domain  F) mediate binding of HNF-4 to Smad3.	bind
80682	5	3471	11	NULL	NULL	0	NULL	statement 3	Protein		mediates					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_3_1279_s_250	12631740	(A-C) Two regions of HNF-4 defined by amino acids 1-49 (domain A/B) and 388-455 (domain  F) mediate binding of HNF-4 to Smad3.	bind
80683	1	3473	11	NULL	NULL	NULL	NULL	[3]CNQX	Chemical		binds to 		two days after lesion			animal	Organism				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_77_2_473_s_97	9472405	(A-C) [3]CNQX binding in an animal two days after lesion; (D-F) [3]MK-801 binding in an animal 30 days after lesion.	bind
80684	2	3473	11	NULL	NULL	0	NULL	[3]MK-801	Chemical		binds to 		30 days after lesion			animal	Organism				NULL		0	NULL	NULL	NULL	gw60_neuroscience_77_2_473_s_97	9472405	(A-C) [3]CNQX binding in an animal two days after lesion; (D-F) [3]MK-801 binding in an animal 30 days after lesion.	bind
7695	1	3474	6	11	NULL	0	NULL	receptor	GP		bind					EGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_3_525_s_180	10069801	(a-d) Receptors bound to EGF-Affi-Gel 15 were phosphorylated with [gamma-32]ATP under autophosphorylation conditions.	bind
7696	2	3474	6	11	NULL	0	NULL	statement 1	GP		undergoes					autophosphorylation	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_3_525_s_180	10069801	(a-d) Receptors bound to EGF-Affi-Gel 15 were phosphorylated with [gamma-32]ATP under autophosphorylation conditions.	bind
10863	2	3474	7	11	NULL	0	NULL	statement 1	GP		undergoes					autophosphorylation	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_3_525_s_180	10069801	(a-d) Receptors bound to EGF-Affi-Gel 15 were phosphorylated with [gamma-32]ATP under autophosphorylation conditions.	bind
52920	1	3474	7	11	NULL	0	NULL	receptor	GP		bind					EGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_3_525_s_180	10069801	(a-d) Receptors bound to EGF-Affi-Gel 15 were phosphorylated with [gamma-32]ATP under autophosphorylation conditions.	bind
80685	1	3474	11	NULL	NULL	0	NULL	Receptors	Protein		binds to 					EGF-Affi-Gel 15	Protein				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_10_3_525_s_180	10069801	(a-d) Receptors bound to EGF-Affi-Gel 15 were phosphorylated with [gamma-32]ATP under autophosphorylation conditions.	bind
80686	1	3478	11	NULL	NULL	NULL	NULL	Apo2L fragment	Protein	recombinant soluble 114 - 281	lacks					polyhistidine tag	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_104_2_155_s_44	10411544	(Although it lacks a polyhistidine tag, the recombinant soluble 114 - 281 Apo2L fragment bound to the Ni-NTA column, probably through endogenous histidine residues.)	bind
80687	2	3478	11	NULL	NULL	0	NULL	Apo2L fragment	Protein	recombinant soluble 114 - 281	binds to 			endogenous histidine residue		Ni-NTA column	LaboratoryExperimentalFactor				NULL		0	NULL	NULL	NULL	gw60_jclininvest_104_2_155_s_44	10411544	(Although it lacks a polyhistidine tag, the recombinant soluble 114 - 281 Apo2L fragment bound to the Ni-NTA column, probably through endogenous histidine residues.)	bind
7733	1	3479	6	11	NULL	0	NULL	Asf1	GP		bind		stably			Rad53	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_1_13_s_92	11172707	(Although perhaps counterintuitive, loss of Mec1 function is not expected to decrease the amount of Asf1 stably bound to Rad53).	bind
14200	2	3479	6	11	NULL	0	NULL	Mec1	GP	loss of;;function of	does not decrease					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_1_13_s_92	11172707	(Although perhaps counterintuitive, loss of Mec1 function is not expected to decrease the amount of Asf1 stably bound to Rad53).	bind
10866	1	3479	7	11	NULL	0	NULL	Asf1	GP		bind		stably			Rad53	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_1_13_s_92	11172707	(Although perhaps counterintuitive, loss of Mec1 function is not expected to decrease the amount of Asf1 stably bound to Rad53).	bind
10867	2	3479	7	11	NULL	0	NULL	Mec1	GP	loss of;;function of	does not decrease					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_1_13_s_92	11172707	(Although perhaps counterintuitive, loss of Mec1 function is not expected to decrease the amount of Asf1 stably bound to Rad53).	bind
80688	1	3479	11	NULL	NULL	0	NULL	Asf1	Protein		binds to 		stably			Rad53	Protein				NULL		0	NULL	NULL	NULL	gw60_molcell_7_1_13_s_92	11172707	(Although perhaps counterintuitive, loss of Mec1 function is not expected to decrease the amount of Asf1 stably bound to Rad53).	bind
80689	2	3479	11	NULL	NULL	0	NULL	Mec1	Protein	loss of function	is not expected to decrease					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_7_1_13_s_92	11172707	(Although perhaps counterintuitive, loss of Mec1 function is not expected to decrease the amount of Asf1 stably bound to Rad53).	bind
7734	1	3480	6	11	NULL	0	NULL	TFIID	GP		does not bind					GST-Gcn4p	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_15_6871_s_102	15254252	(Although Taf9p and Taf12p are shared by SAGA and TFIID, we showed previously that TFIID does not bind to GST-Gcn4p in these assays ( ).	bind
10868	1	3480	7	11	NULL	0	NULL	TFIID 	GP		does not bind					GST-Gcn4p	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_15_6871_s_102	15254252	(Although Taf9p and Taf12p are shared by SAGA and TFIID, we showed previously that TFIID does not bind to GST-Gcn4p in these assays ( ).	bind
80690	1	3480	11	NULL	NULL	0	NULL	TFIID	Protein		does not bind to					GST-Gcn4p	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_15_6871_s_102	15254252	(Although Taf9p and Taf12p are shared by SAGA and TFIID, we showed previously that TFIID does not bind to GST-Gcn4p in these assays ( ).	bind
80691	2	3480	11	NULL	NULL	0	NULL	Taf9p	Protein		shared by					SAGA	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_15_6871_s_102	15254252	(Although Taf9p and Taf12p are shared by SAGA and TFIID, we showed previously that TFIID does not bind to GST-Gcn4p in these assays ( ).	bind
80692	3	3480	11	NULL	NULL	0	NULL	Taf9p	Protein		shared by					TFIID	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_15_6871_s_102	15254252	(Although Taf9p and Taf12p are shared by SAGA and TFIID, we showed previously that TFIID does not bind to GST-Gcn4p in these assays ( ).	bind
80693	4	3480	11	NULL	NULL	0	NULL	Taf12p	Protein		shared by					SAGA	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_15_6871_s_102	15254252	(Although Taf9p and Taf12p are shared by SAGA and TFIID, we showed previously that TFIID does not bind to GST-Gcn4p in these assays ( ).	bind
80694	5	3480	11	NULL	NULL	0	NULL	Taf12p	Protein		shared by					TFIID	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_15_6871_s_102	15254252	(Although Taf9p and Taf12p are shared by SAGA and TFIID, we showed previously that TFIID does not bind to GST-Gcn4p in these assays ( ).	bind
7735	1	3485	6	11	NULL	0	NULL	Arf-GTPase-activating protein 1	GP		bind		constitutively			CIN85	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_39_28919_s_419	16895919	(Arf-GTPase-activating protein 1) constitutively binds to CIN85 and induces an increase in EGF receptor recycling ( ,  ).	bind
7736	2	3485	6	11	NULL	0	NULL	statement 1	Process		increase					EGF receptor	GP	recycling of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_39_28919_s_419	16895919	(Arf-GTPase-activating protein 1) constitutively binds to CIN85 and induces an increase in EGF receptor recycling ( ,  ).	bind
10869	1	3485	7	11	NULL	0	NULL	Arf-GTPase-activating protein 1	GP		bind		constitutively			CIN85	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_39_28919_s_419	16895919	(Arf-GTPase-activating protein 1) constitutively binds to CIN85 and induces an increase in EGF receptor recycling ( ,  ).	bind
10870	2	3485	7	11	NULL	0	NULL	statement 1	Process		increase					EGF receptor	GP	recycling of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_39_28919_s_419	16895919	(Arf-GTPase-activating protein 1) constitutively binds to CIN85 and induces an increase in EGF receptor recycling ( ,  ).	bind
80695	1	3485	11	NULL	NULL	0	NULL	Arf-GTPase-activating protein 1	Protein		binds to 					CIN85	Protein				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_39_28919_s_419	16895919	(Arf-GTPase-activating protein 1) constitutively binds to CIN85 and induces an increase in EGF receptor recycling ( ,  ).	bind
80696	2	3485	11	NULL	NULL	0	NULL	statement 1	Process		induces					recycling	Process	EGF receptor			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_39_28919_s_419	16895919	(Arf-GTPase-activating protein 1) constitutively binds to CIN85 and induces an increase in EGF receptor recycling ( ,  ).	bind
7737	1	3486	6	11	NULL	0	NULL	Grb2	GP		bind					PTPalpha	GP	endogenous;;WT			NULL	Neo control cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_24_21922_s_181	11923305	(As previously noted, Grb2 bound a larger fraction of endogenous WT PTPalpha ( i.e. in the Neo control cells) than overexpressed WT PTPalpha.	bind
52940	2	3486	6	11	NULL	0	NULL	Grb2	GP		bind					PTPalpha	GP	overexpressed;;WT			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_24_21922_s_181	11923305	(As previously noted, Grb2 bound a larger fraction of endogenous WT PTPalpha ( i.e. in the Neo control cells) than overexpressed WT PTPalpha.	bind
52941	3	3486	6	11	NULL	0	NULL	statement 1	Process		greater than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_24_21922_s_181	11923305	(As previously noted, Grb2 bound a larger fraction of endogenous WT PTPalpha ( i.e. in the Neo control cells) than overexpressed WT PTPalpha.	bind
10871	1	3486	7	11	NULL	0	NULL	Grb2	GP		bind					PTPalpha	GP	endogenous;; WT			NULL	in the Neo control cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_24_21922_s_181	11923305	(As previously noted, Grb2 bound a larger fraction of endogenous WT PTPalpha ( i.e. in the Neo control cells) than overexpressed WT PTPalpha.	bind
10872	2	3486	7	11	NULL	0	NULL	Grb2	GP		bind					PTPalpha	GP	overexpressed;;WT			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_24_21922_s_181	11923305	(As previously noted, Grb2 bound a larger fraction of endogenous WT PTPalpha ( i.e. in the Neo control cells) than overexpressed WT PTPalpha.	bind
10873	3	3486	7	11	NULL	0	NULL	statement 1	Process		greater than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_24_21922_s_181	11923305	(As previously noted, Grb2 bound a larger fraction of endogenous WT PTPalpha ( i.e. in the Neo control cells) than overexpressed WT PTPalpha.	bind
80697	1	3486	11	NULL	NULL	0	NULL	Grb2	Protein		binds to 					WT PTPalpha	Protein	endogenous			NULL	 Neo control cells	0	NULL	NULL	NULL	gw60_jbiolchem_277_24_21922_s_181	11923305	(As previously noted, Grb2 bound a larger fraction of endogenous WT PTPalpha ( i.e. in the Neo control cells) than overexpressed WT PTPalpha.	bind
80698	2	3486	11	NULL	NULL	0	NULL	Grb2	Protein		binds to 					WT PTPalpha	Protein	overexpressed			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_24_21922_s_181	11923305	(As previously noted, Grb2 bound a larger fraction of endogenous WT PTPalpha ( i.e. in the Neo control cells) than overexpressed WT PTPalpha.	bind
7738	1	3487	6	11	NULL	0	NULL	lidocaine	Chemical		bind					IS	Process				NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_66_3_648_s_213	15322257	(As shown in  Fig. 4, the  KD for lidocaine binding to IS is similar to the  KD for lidocaine binding to IM).	bind
7739	2	3487	6	11	NULL	0	NULL	lidocaine	Chemical		bind					IM	Process				NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_66_3_648_s_213	15322257	(As shown in  Fig. 4, the  KD for lidocaine binding to IS is similar to the  KD for lidocaine binding to IM).	bind
10885	1	3487	7	11	NULL	0	NULL	lidocaine	Chemical		bind					IS 	Process				NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_66_3_648_s_213	15322257	(As shown in  Fig. 4, the  KD for lidocaine binding to IS is similar to the  KD for lidocaine binding to IM).	bind
10886	2	3487	7	11	NULL	0	NULL	lidocaine	Chemical		bind					IM	Process				NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_66_3_648_s_213	15322257	(As shown in  Fig. 4, the  KD for lidocaine binding to IS is similar to the  KD for lidocaine binding to IM).	bind
80699	1	3487	11	NULL	NULL	0	NULL	lidocaine	Chemical		binds to 					IS	LaboratoryExperimentalFactor				NULL		0	NULL	NULL	NULL	gw70_molpharmacol_66_3_648_s_213	15322257	(As shown in  Fig. 4, the  KD for lidocaine binding to IS is similar to the  KD for lidocaine binding to IM).	bind
80700	2	3487	11	NULL	NULL	0	NULL	lidocaine	Chemical		binds to 					IM	LaboratoryExperimentalFactor				NULL		0	NULL	NULL	NULL	gw70_molpharmacol_66_3_648_s_213	15322257	(As shown in  Fig. 4, the  KD for lidocaine binding to IS is similar to the  KD for lidocaine binding to IM).	bind
80701	3	3487	11	NULL	NULL	0	NULL	statement 1	Process	KD	is similar to					statement 2	Process	KD			NULL		0	NULL	NULL	NULL	gw70_molpharmacol_66_3_648_s_213	15322257	(As shown in  Fig. 4, the  KD for lidocaine binding to IS is similar to the  KD for lidocaine binding to IM).	bind
7740	1	3489	6	11	NULL	0	NULL	enolase	GP	A. hydrophila	bind					plasminogen	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_microbpathogenesis_34_4_195_s_124	12668143	(B and C)  A. hydrophila enolase binds with human plasminogen based on sandwich Western blot analysis.	bind
10888	1	3489	7	11	NULL	0	NULL	enolase	GP	A. hydrophila	bind					plasminogen	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_microbpathogenesis_34_4_195_s_124	12668143	(B and C)  A. hydrophila enolase binds with human plasminogen based on sandwich Western blot analysis.	bind
80706	1	3489	11	NULL	NULL	0	NULL	enolase	Protein	A. hydrophila	binds to 					plasminogen	Protein	human			NULL	sandwich Western blot analysis	0	NULL	NULL	NULL	gw60_microbpathogenesis_34_4_195_s_124	12668143	(B and C)  A. hydrophila enolase binds with human plasminogen based on sandwich Western blot analysis.	bind
80708	1	3490	11	NULL	NULL	0	NULL	70Z/3 cells	cell		stimulated with					LPS	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_14_6488_s_163	15226448	(B and C) 70Z/3 cells were stimulated with LPS or PMA (B) or UV light (C) for the  times indicated, and whole-cell extracts were analyzed for NF-kappaB and AP-1 DNA binding and JunB, JunD, and p65 expression levels by Western blotting.	bind
80709	2	3490	11	NULL	NULL	0	NULL	70Z/3 cells	cell		stimulated with					PMA	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_14_6488_s_163	15226448	(B and C) 70Z/3 cells were stimulated with LPS or PMA (B) or UV light (C) for the  times indicated, and whole-cell extracts were analyzed for NF-kappaB and AP-1 DNA binding and JunB, JunD, and p65 expression levels by Western blotting.	bind
80710	3	3490	11	NULL	NULL	0	NULL	70Z/3 cells	cell		stimulated with					UV light	LaboratoryExperimentalFactor				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_14_6488_s_163	15226448	(B and C) 70Z/3 cells were stimulated with LPS or PMA (B) or UV light (C) for the  times indicated, and whole-cell extracts were analyzed for NF-kappaB and AP-1 DNA binding and JunB, JunD, and p65 expression levels by Western blotting.	bind
80711	4	3490	11	NULL	NULL	0	NULL	DNA	NucleicAcidSubstance		binds to 					NF-kappaB	Protein				NULL	70Z/3 whole-cell extract	0	NULL	NULL	NULL	gw70_molcellbiol_24_14_6488_s_163	15226448	(B and C) 70Z/3 cells were stimulated with LPS or PMA (B) or UV light (C) for the  times indicated, and whole-cell extracts were analyzed for NF-kappaB and AP-1 DNA binding and JunB, JunD, and p65 expression levels by Western blotting.	bind
80712	5	3490	11	NULL	NULL	0	NULL	DNA	NucleicAcidSubstance		binds to 					AP-1	Protein				NULL	70Z/3 whole-cell extract	0	NULL	NULL	NULL	gw70_molcellbiol_24_14_6488_s_163	15226448	(B and C) 70Z/3 cells were stimulated with LPS or PMA (B) or UV light (C) for the  times indicated, and whole-cell extracts were analyzed for NF-kappaB and AP-1 DNA binding and JunB, JunD, and p65 expression levels by Western blotting.	bind
80713	6	3490	11	NULL	NULL	0	NULL	70Z/3 cells	cell	whole-cell extract	express					JunB	Gene				NULL	Western blotting	0	NULL	NULL	NULL	gw70_molcellbiol_24_14_6488_s_163	15226448	(B and C) 70Z/3 cells were stimulated with LPS or PMA (B) or UV light (C) for the  times indicated, and whole-cell extracts were analyzed for NF-kappaB and AP-1 DNA binding and JunB, JunD, and p65 expression levels by Western blotting.	bind
80714	7	3490	11	NULL	NULL	0	NULL	70Z/3 cells	cell	whole-cell extract	express					JunD	Gene				NULL	Western blotting	0	NULL	NULL	NULL	gw70_molcellbiol_24_14_6488_s_163	15226448	(B and C) 70Z/3 cells were stimulated with LPS or PMA (B) or UV light (C) for the  times indicated, and whole-cell extracts were analyzed for NF-kappaB and AP-1 DNA binding and JunB, JunD, and p65 expression levels by Western blotting.	bind
80715	8	3490	11	NULL	NULL	0	NULL	70Z/3 cells	cell	whole-cell extract	express					p65	Gene				NULL	Western blotting	0	NULL	NULL	NULL	gw70_molcellbiol_24_14_6488_s_163	15226448	(B and C) 70Z/3 cells were stimulated with LPS or PMA (B) or UV light (C) for the  times indicated, and whole-cell extracts were analyzed for NF-kappaB and AP-1 DNA binding and JunB, JunD, and p65 expression levels by Western blotting.	bind
7743	1	3491	6	11	NULL	0	NULL	ATF6alpha	GP		bind									ERSE-CC	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_4_1239_s_185	11158310	(B and C) Binding of ATF6alpha(B) and ATF6beta (C) in the presence of NF-Y to resin carrying ERSE-CC.	bind
7744	2	3491	6	11	NULL	0	NULL	ATF6beta	GP		bind									ERSE-CC	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_4_1239_s_185	11158310	(B and C) Binding of ATF6alpha(B) and ATF6beta (C) in the presence of NF-Y to resin carrying ERSE-CC.	bind
7745	3	3491	6	11	NULL	0	NULL	statement 1	Process		occurs in presence of					NF-Y	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_4_1239_s_185	11158310	(B and C) Binding of ATF6alpha(B) and ATF6beta (C) in the presence of NF-Y to resin carrying ERSE-CC.	bind
7746	4	3491	6	11	NULL	0	NULL	statement 2	Process		occurs in presence of					NF-Y	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_4_1239_s_185	11158310	(B and C) Binding of ATF6alpha(B) and ATF6beta (C) in the presence of NF-Y to resin carrying ERSE-CC.	bind
10894	1	3491	7	11	NULL	0	NULL	ATF6alpha	GP		bind									ERSE-CC	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_4_1239_s_185	11158310	(B and C) Binding of ATF6alpha(B) and ATF6beta (C) in the presence of NF-Y to resin carrying ERSE-CC.	bind
10895	2	3491	7	11	NULL	0	NULL	ATF6beta	GP		bind									ERSE-CC	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_4_1239_s_185	11158310	(B and C) Binding of ATF6alpha(B) and ATF6beta (C) in the presence of NF-Y to resin carrying ERSE-CC.	bind
52942	3	3491	7	11	NULL	0	NULL	statement 1	Process		occurs in presence of					NF-Y	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_4_1239_s_185	11158310	(B and C) Binding of ATF6alpha(B) and ATF6beta (C) in the presence of NF-Y to resin carrying ERSE-CC.	bind
52944	4	3491	7	11	NULL	0	NULL	statement 2	Process		occurs in presence of					NF-Y	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_4_1239_s_185	11158310	(B and C) Binding of ATF6alpha(B) and ATF6beta (C) in the presence of NF-Y to resin carrying ERSE-CC.	bind
80716	1	3491	11	NULL	NULL	0	NULL	ATF6alpha	Protein		binds to 					ERSE-CC	NucleicAcidSubstance	resin carrying			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1239_s_185	11158310	(B and C) Binding of ATF6alpha(B) and ATF6beta (C) in the presence of NF-Y to resin carrying ERSE-CC.	bind
80717	2	3491	11	NULL	NULL	0	NULL	ATF6beta	Protein		binds to 					ERSE-CC	NucleicAcidSubstance	resin carrying			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1239_s_185	11158310	(B and C) Binding of ATF6alpha(B) and ATF6beta (C) in the presence of NF-Y to resin carrying ERSE-CC.	bind
80719	3	3491	11	NULL	NULL	0	NULL	statement 1	Process		occurs in the presence of					NF-Y	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1239_s_185	11158310	(B and C) Binding of ATF6alpha(B) and ATF6beta (C) in the presence of NF-Y to resin carrying ERSE-CC.	bind
80720	4	3491	11	NULL	NULL	0	NULL	statement 2	Process		occurs in the presence of					NF-Y	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1239_s_185	11158310	(B and C) Binding of ATF6alpha(B) and ATF6beta (C) in the presence of NF-Y to resin carrying ERSE-CC.	bind
7747	1	3492	6	11	NULL	0	NULL	NF-Y	GP		bind					HLA-DRA	GP			Y box	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6495_s_290	11533238	(B and C) Binding of NF-Y to the HLA-DRA Y box and YY1 to the +62/+72 HLA-DRA YY1 binding element is not affected by treatment of cells with HDAC inhibitors.	bind
7748	2	3492	6	11	NULL	0	NULL	NF-Y	GP		bind					HLA-DRA	GP			YY1 binding element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6495_s_290	11533238	(B and C) Binding of NF-Y to the HLA-DRA Y box and YY1 to the +62/+72 HLA-DRA YY1 binding element is not affected by treatment of cells with HDAC inhibitors.	bind
7797	3	3492	6	11	NULL	0	NULL	HDAC inhibitors	Chemical		have no effect on					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6495_s_290	11533238	(B and C) Binding of NF-Y to the HLA-DRA Y box and YY1 to the +62/+72 HLA-DRA YY1 binding element is not affected by treatment of cells with HDAC inhibitors.	bind
7798	4	3492	6	11	NULL	0	NULL	HDAC inhibitors	Chemical		have no effect on					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6495_s_290	11533238	(B and C) Binding of NF-Y to the HLA-DRA Y box and YY1 to the +62/+72 HLA-DRA YY1 binding element is not affected by treatment of cells with HDAC inhibitors.	bind
10900	1	3492	7	11	NULL	0	NULL	NF-Y	GP		bind					HLA-DRA	GP			Y box	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6495_s_290	11533238	(B and C) Binding of NF-Y to the HLA-DRA Y box and YY1 to the +62/+72 HLA-DRA YY1 binding element is not affected by treatment of cells with HDAC inhibitors.	bind
10906	2	3492	7	11	NULL	0	NULL	YY1	GP		bind					HLA-DRA	GP			YY1 binding element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6495_s_290	11533238	(B and C) Binding of NF-Y to the HLA-DRA Y box and YY1 to the +62/+72 HLA-DRA YY1 binding element is not affected by treatment of cells with HDAC inhibitors.	bind
10907	3	3492	7	11	NULL	0	NULL	statement 1	Process		is not affected by 					HDAC inhibitors	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6495_s_290	11533238	(B and C) Binding of NF-Y to the HLA-DRA Y box and YY1 to the +62/+72 HLA-DRA YY1 binding element is not affected by treatment of cells with HDAC inhibitors.	bind
10908	4	3492	7	11	NULL	0	NULL	statement 2	Process		is not affected by					HDAC inhibitors	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6495_s_290	11533238	(B and C) Binding of NF-Y to the HLA-DRA Y box and YY1 to the +62/+72 HLA-DRA YY1 binding element is not affected by treatment of cells with HDAC inhibitors.	bind
80721	1	3492	11	NULL	NULL	NULL	NULL	NF-Y	Protein		binds to 					HLA-DRA	Gene	Y box			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6495_s_290	11533238	(B and C) Binding of NF-Y to the HLA-DRA Y box and YY1 to the +62/+72 HLA-DRA YY1 binding element is not affected by treatment of cells with HDAC inhibitors.	bind
80722	2	3492	11	NULL	NULL	0	NULL	YY1	Protein		binds to 					HLA-DRA	Gene				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_19_6495_s_290	11533238	(B and C) Binding of NF-Y to the HLA-DRA Y box and YY1 to the +62/+72 HLA-DRA YY1 binding element is not affected by treatment of cells with HDAC inhibitors.	bind
80723	3	3492	11	NULL	NULL	0	NULL	HLA-DRA	Gene		is not affected by				YY1 binding element	inhibitors	Chemical	HDAC			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_19_6495_s_290	11533238	(B and C) Binding of NF-Y to the HLA-DRA Y box and YY1 to the +62/+72 HLA-DRA YY1 binding element is not affected by treatment of cells with HDAC inhibitors.	bind
7799	1	3493	6	11	NULL	0	NULL	TFIIB	GP	binding of	is dependent on					Swi5	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_6_1213_s_91	11430824	(B and C) Binding of TFIIB and Kin28 depends on Swi5.	bind
7800	2	3493	6	11	NULL	0	NULL	Kin28	GP	binding of	is dependent on					Swi5	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_6_1213_s_91	11430824	(B and C) Binding of TFIIB and Kin28 depends on Swi5.	bind
10910	1	3493	7	11	NULL	0	NULL	TFIIB	GP	binding of	is dependent on					Swi5	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_6_1213_s_91	11430824	(B and C) Binding of TFIIB and Kin28 depends on Swi5.	bind
10912	2	3493	7	11	NULL	0	NULL	Kin28 	GP	binding of	is dependent on					Swi5	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_6_1213_s_91	11430824	(B and C) Binding of TFIIB and Kin28 depends on Swi5.	bind
80724	1	3493	11	NULL	NULL	0	NULL	Binding	MolecularProcess	 TFIIB	depends on					Swi5	Protein				NULL		0	NULL	NULL	NULL	gw60_molcell_7_6_1213_s_91	11430824	(B and C) Binding of TFIIB and Kin28 depends on Swi5.	bind
80725	2	3493	11	NULL	NULL	0	NULL	Binding	MolecularProcess	Kin28	depends on					Swi5	Protein				NULL		0	NULL	NULL	NULL	gw60_molcell_7_6_1213_s_91	11430824	(B and C) Binding of TFIIB and Kin28 depends on Swi5.	bind
7801	1	3494	6	11	NULL	0	NULL	RXR-TR heterodimer	GP		bind							specific		TRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_252	10891484	(B and C) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-TR heterodimer bound to a specific TRE.	bind
7802	2	3494	6	11	NULL	0	NULL	TRAP220	GP		bind			RBD		statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_252	10891484	(B and C) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-TR heterodimer bound to a specific TRE.	bind
7804	3	3494	6	11	NULL	0	NULL				is necessary for			RBD-1		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_252	10891484	(B and C) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-TR heterodimer bound to a specific TRE.	bind
14598	4	3494	6	11	NULL	0	NULL				is necessary for			RBD-2		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_252	10891484	(B and C) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-TR heterodimer bound to a specific TRE.	bind
14599	5	3494	6	11	NULL	0	NULL	statement 3	Process		is simultaneous with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_252	10891484	(B and C) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-TR heterodimer bound to a specific TRE.	bind
14600	7	3494	6	11	NULL	0	NULL			proper spacing of	is necessary for			RBD-1		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_252	10891484	(B and C) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-TR heterodimer bound to a specific TRE.	bind
17772	8	3494	6	11	NULL	0	NULL			proper spacing of	is necessary for			RBD-2		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_252	10891484	(B and C) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-TR heterodimer bound to a specific TRE.	bind
17773	9	3494	6	11	NULL	0	NULL	statement 7	Process		is simultaneous with					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_252	10891484	(B and C) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-TR heterodimer bound to a specific TRE.	bind
10915	1	3494	7	11	NULL	0	NULL	RXR-TR heterodimer	GP		bind							specific		TRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_252	10891484	(B and C) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-TR heterodimer bound to a specific TRE.	bind
10916	2	3494	7	11	NULL	0	NULL	TRAP220 	GP		bind			RBD		statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_252	10891484	(B and C) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-TR heterodimer bound to a specific TRE.	bind
10917	3	3494	7	11	NULL	0	NULL				is necessary for			RBD-1		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_252	10891484	(B and C) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-TR heterodimer bound to a specific TRE.	bind
10918	4	3494	7	11	NULL	0	NULL				is necessary for			RBD-2		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_252	10891484	(B and C) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-TR heterodimer bound to a specific TRE.	bind
15014	5	3494	7	11	NULL	0	NULL	statement 3	Process		is simultaneous with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_252	10891484	(B and C) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-TR heterodimer bound to a specific TRE.	bind
15015	6	3494	7	11	NULL	0	NULL			proper spacing of	is necessary for			RBD-1		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_252	10891484	(B and C) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-TR heterodimer bound to a specific TRE.	bind
15016	7	3494	7	11	NULL	0	NULL			proper spacing of	is necessary for			RBD-2		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_252	10891484	(B and C) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-TR heterodimer bound to a specific TRE.	bind
15017	8	3494	7	11	NULL	0	NULL	statement 6	Process		is simultaneous with					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_252	10891484	(B and C) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-TR heterodimer bound to a specific TRE.	bind
80726	1	3494	11	NULL	NULL	0	NULL	RXR-TR	Protein		is a type of 					heterodimer	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_252	10891484	(B and C) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-TR heterodimer bound to a specific TRE.	bind
80727	2	3494	11	NULL	NULL	NULL	NULL	RXR-TR heterodimer	GeneOrProtein		binds to 					 TRE	NucleicAcidSubstance	specific			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_252	10891484	(B and C) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-TR heterodimer bound to a specific TRE.	bind
80728	3	3494	11	NULL	NULL	0	NULL	TRAP220 RBD	Protein		binds to 					statement 2	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_252	10891484	(B and C) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-TR heterodimer bound to a specific TRE.	bind
80729	4	3494	11	NULL	NULL	0	NULL	RBD-1	Protein	presence;;proper spacing	necessary for					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_252	10891484	(B and C) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-TR heterodimer bound to a specific TRE.	bind
80730	5	3494	11	NULL	NULL	0	NULL	RBD-2 	Protein	presence;;proper spacing	necessary for					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_252	10891484	(B and C) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-TR heterodimer bound to a specific TRE.	bind
7805	1	3495	6	11	NULL	0	NULL	Gsp1p-GTP	GP		bind					Los1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_11_6374_s_306	9774653	(B and C) Cooperative binding of Gsp1p-GTP and tRNA to Los1p.	bind
7807	2	3495	6	11	NULL	0	NULL	tRNA	NucleicAcid		bind					Los1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_11_6374_s_306	9774653	(B and C) Cooperative binding of Gsp1p-GTP and tRNA to Los1p.	bind
7808	3	3495	6	11	NULL	0	NULL	statement 1	Process		acts in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_11_6374_s_306	9774653	(B and C) Cooperative binding of Gsp1p-GTP and tRNA to Los1p.	bind
10919	1	3495	7	11	NULL	0	NULL	Gsp1p-GTP	GP		bind					Los1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_11_6374_s_306	9774653	(B and C) Cooperative binding of Gsp1p-GTP and tRNA to Los1p.	bind
10920	2	3495	7	11	NULL	0	NULL	tRNA	NucleicAcid		bind					Los1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_11_6374_s_306	9774653	(B and C) Cooperative binding of Gsp1p-GTP and tRNA to Los1p.	bind
10921	3	3495	7	11	NULL	0	NULL	statement 1	Process		occurs in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_11_6374_s_306	9774653	(B and C) Cooperative binding of Gsp1p-GTP and tRNA to Los1p.	bind
80731	1	3495	11	NULL	NULL	0	NULL	Gsp1p-GTP	Protein		binds to 		cooperatively			Los1p	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_11_6374_s_306	9774653	(B and C) Cooperative binding of Gsp1p-GTP and tRNA to Los1p.	bind
80732	2	3495	11	NULL	NULL	0	NULL	tRNA	NucleicAcidSubstance		binds to 		cooperatively			Los1p	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_11_6374_s_306	9774653	(B and C) Cooperative binding of Gsp1p-GTP and tRNA to Los1p.	bind
7810	1	3496	6	11	NULL	0	NULL	GST-Hairy derivatives	GP		bind					Gro	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_2080_s_156	10022895	(B and C) Expression of HairyWRPW (B) and HairyGEH-17 (C) under the control of the  hb promoter causes efficient repression of  Sxl. (D) Binding of GST-Hairy derivatives to Gro in vitro.	bind
7812	2	3496	6	11	NULL	0	NULL	hb	GP		controls				promoter	HairyWRPW	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_2080_s_156	10022895	(B and C) Expression of HairyWRPW (B) and HairyGEH-17 (C) under the control of the  hb promoter causes efficient repression of  Sxl. (D) Binding of GST-Hairy derivatives to Gro in vitro.	bind
7813	3	3496	6	11	NULL	0	NULL	hb	GP		controls				promoter	HairyGEH-17	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_2080_s_156	10022895	(B and C) Expression of HairyWRPW (B) and HairyGEH-17 (C) under the control of the  hb promoter causes efficient repression of  Sxl. (D) Binding of GST-Hairy derivatives to Gro in vitro.	bind
7814	4	3496	6	11	NULL	0	NULL	HairyWRPW	GP	expression of	repress		efficiently			Sxl	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_2080_s_156	10022895	(B and C) Expression of HairyWRPW (B) and HairyGEH-17 (C) under the control of the  hb promoter causes efficient repression of  Sxl. (D) Binding of GST-Hairy derivatives to Gro in vitro.	bind
7815	5	3496	6	11	NULL	0	NULL	HairyGEH-17	GP	expression of	repress		efficiently			Sxl	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_2080_s_156	10022895	(B and C) Expression of HairyWRPW (B) and HairyGEH-17 (C) under the control of the  hb promoter causes efficient repression of  Sxl. (D) Binding of GST-Hairy derivatives to Gro in vitro.	bind
10922	1	3496	7	11	NULL	0	NULL	GST-Hairy derivatives	GP		bind					Gro	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_2080_s_156	10022895	(B and C) Expression of HairyWRPW (B) and HairyGEH-17 (C) under the control of the  hb promoter causes efficient repression of  Sxl. (D) Binding of GST-Hairy derivatives to Gro in vitro.	bind
10923	2	3496	7	11	NULL	0	NULL	HairyWRPW	GP	expression of	repress		efficiently			Sxl	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_2080_s_156	10022895	(B and C) Expression of HairyWRPW (B) and HairyGEH-17 (C) under the control of the  hb promoter causes efficient repression of  Sxl. (D) Binding of GST-Hairy derivatives to Gro in vitro.	bind
10924	3	3496	7	11	NULL	0	NULL	HairyGEH-17	GP	expression of	repress		efficiently			Sxl	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_2080_s_156	10022895	(B and C) Expression of HairyWRPW (B) and HairyGEH-17 (C) under the control of the  hb promoter causes efficient repression of  Sxl. (D) Binding of GST-Hairy derivatives to Gro in vitro.	bind
10925	4	3496	7	11	NULL	0	NULL	statement 2	Process		occus under					hb	GP	the control of		promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_2080_s_156	10022895	(B and C) Expression of HairyWRPW (B) and HairyGEH-17 (C) under the control of the  hb promoter causes efficient repression of  Sxl. (D) Binding of GST-Hairy derivatives to Gro in vitro.	bind
10926	5	3496	7	11	NULL	0	NULL	statement 3	Process		occurs under 					hb	GP	the control of		promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_2080_s_156	10022895	(B and C) Expression of HairyWRPW (B) and HairyGEH-17 (C) under the control of the  hb promoter causes efficient repression of  Sxl. (D) Binding of GST-Hairy derivatives to Gro in vitro.	bind
80733	1	3496	11	NULL	NULL	0	NULL	GST-Hairy	Protein	derivatives	binds to 					Gro	Protein				NULL	in vitro	0	NULL	NULL	NULL	gw60_molcellbiol_19_3_2080_s_156	10022895	(B and C) Expression of HairyWRPW (B) and HairyGEH-17 (C) under the control of the  hb promoter causes efficient repression of  Sxl. (D) Binding of GST-Hairy derivatives to Gro in vitro.	bind
80734	2	3496	11	NULL	NULL	0	NULL	hb promoter	NucleicAcidSubstance		controls					Expression	MolecularProcess	HairyWRPW			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_3_2080_s_156	10022895	(B and C) Expression of HairyWRPW (B) and HairyGEH-17 (C) under the control of the  hb promoter causes efficient repression of  Sxl. (D) Binding of GST-Hairy derivatives to Gro in vitro.	bind
80735	3	3496	11	NULL	NULL	0	NULL	statement 2	Process		repress					Sxl	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_3_2080_s_156	10022895	(B and C) Expression of HairyWRPW (B) and HairyGEH-17 (C) under the control of the  hb promoter causes efficient repression of  Sxl. (D) Binding of GST-Hairy derivatives to Gro in vitro.	bind
80736	4	3496	11	NULL	NULL	0	NULL	hb promoter	NucleicAcidSubstance		controls					Expression	MolecularProcess	HairyGEH-17			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_3_2080_s_156	10022895	(B and C) Expression of HairyWRPW (B) and HairyGEH-17 (C) under the control of the  hb promoter causes efficient repression of  Sxl. (D) Binding of GST-Hairy derivatives to Gro in vitro.	bind
80737	5	3496	11	NULL	NULL	0	NULL	statement 4	Process		repress					Sxl	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_3_2080_s_156	10022895	(B and C) Expression of HairyWRPW (B) and HairyGEH-17 (C) under the control of the  hb promoter causes efficient repression of  Sxl. (D) Binding of GST-Hairy derivatives to Gro in vitro.	bind
7816	1	3497	6	11	NULL	0	NULL	Flo8	GP		bind					UAS2-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_194	15485921	(B and C) Flo8 and Mss11  binding to UAS2-1 requires Ste12 and Tec1.	bind
7817	2	3497	6	11	NULL	0	NULL	Mss11	GP		bind					UAS2-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_194	15485921	(B and C) Flo8 and Mss11  binding to UAS2-1 requires Ste12 and Tec1.	bind
7818	3	3497	6	11	NULL	0	NULL	statement 1	Process		requires					Ste12	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_194	15485921	(B and C) Flo8 and Mss11  binding to UAS2-1 requires Ste12 and Tec1.	bind
7819	4	3497	6	11	NULL	0	NULL	statement 1	Process		requires					Tec1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_194	15485921	(B and C) Flo8 and Mss11  binding to UAS2-1 requires Ste12 and Tec1.	bind
7820	5	3497	6	11	NULL	0	NULL	statement 2	Process		requires					Ste12	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_194	15485921	(B and C) Flo8 and Mss11  binding to UAS2-1 requires Ste12 and Tec1.	bind
7822	6	3497	6	11	NULL	0	NULL	statement 2	Process		requires					Tec1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_194	15485921	(B and C) Flo8 and Mss11  binding to UAS2-1 requires Ste12 and Tec1.	bind
10927	1	3497	7	11	NULL	0	NULL	Flo8	GP		bind					UAS2-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_194	15485921	(B and C) Flo8 and Mss11  binding to UAS2-1 requires Ste12 and Tec1.	bind
10928	2	3497	7	11	NULL	0	NULL	Mss11	GP		bind					UAS2-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_194	15485921	(B and C) Flo8 and Mss11  binding to UAS2-1 requires Ste12 and Tec1.	bind
10929	3	3497	7	11	NULL	0	NULL	statement 1	Process		requires					Ste12	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_194	15485921	(B and C) Flo8 and Mss11  binding to UAS2-1 requires Ste12 and Tec1.	bind
10930	4	3497	7	11	NULL	0	NULL	statement 1	Process		requires					Tec1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_194	15485921	(B and C) Flo8 and Mss11  binding to UAS2-1 requires Ste12 and Tec1.	bind
10931	5	3497	7	11	NULL	0	NULL	statement 2	Process		requires					Ste12	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_194	15485921	(B and C) Flo8 and Mss11  binding to UAS2-1 requires Ste12 and Tec1.	bind
10932	6	3497	7	11	NULL	0	NULL	statement 2	Process		requires					Tec1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_194	15485921	(B and C) Flo8 and Mss11  binding to UAS2-1 requires Ste12 and Tec1.	bind
80738	1	3497	11	NULL	NULL	NULL	NULL	Flo8	GeneOrProtein		binds to 					UAS2-1	NucleicAcidSubstance				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_194	15485921	(B and C) Flo8 and Mss11  binding to UAS2-1 requires Ste12 and Tec1.	bind
80739	2	3497	11	NULL	NULL	0	NULL	Mss11	GeneOrProtein		binds to 					UAS2-1	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_194	15485921	(B and C) Flo8 and Mss11  binding to UAS2-1 requires Ste12 and Tec1.	bind
80740	3	3497	11	NULL	NULL	0	NULL	statement 1	Process		requires					Ste12	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_194	15485921	(B and C) Flo8 and Mss11  binding to UAS2-1 requires Ste12 and Tec1.	bind
80741	4	3497	11	NULL	NULL	NULL	NULL	statement 1	Process		requires					Tec1	GeneOrProtein				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_194	15485921	(B and C) Flo8 and Mss11  binding to UAS2-1 requires Ste12 and Tec1.	bind
80742	5	3497	11	NULL	NULL	0	NULL	statement 2	Process		requires					Ste12	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_194	15485921	(B and C) Flo8 and Mss11  binding to UAS2-1 requires Ste12 and Tec1.	bind
80743	6	3497	11	NULL	NULL	0	NULL	statement 2	Process		requires					Tec1	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_194	15485921	(B and C) Flo8 and Mss11  binding to UAS2-1 requires Ste12 and Tec1.	bind
7825	1	3499	6	11	NULL	0	NULL	eIF2B subunits	GP		bind					eIF2alpha	GP	phosphorylated			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3063_s_290	15798194	(B and C) Mutations of eIF2alpha residues near and remote from Ser51 impair binding of eIF2B subunits to phosphorylated  eIF2alpha.	bind
7827	2	3499	6	11	NULL	0	NULL	eIF2alpha	GP	mutation of	impair 			 near Ser51		statement 1	Process	binding of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3063_s_290	15798194	(B and C) Mutations of eIF2alpha residues near and remote from Ser51 impair binding of eIF2B subunits to phosphorylated  eIF2alpha.	bind
14201	3	3499	6	11	NULL	0	NULL	eIF2alpha	GP	mutation of	impair			remote from Ser51		statement 1	Process	binding of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3063_s_290	15798194	(B and C) Mutations of eIF2alpha residues near and remote from Ser51 impair binding of eIF2B subunits to phosphorylated  eIF2alpha.	bind
10933	1	3499	7	11	NULL	0	NULL	eIF2B subunits	GP		bind					eIF2alpha	GP	phosphorylated			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3063_s_290	15798194	(B and C) Mutations of eIF2alpha residues near and remote from Ser51 impair binding of eIF2B subunits to phosphorylated  eIF2alpha.	bind
10934	2	3499	7	11	NULL	0	NULL	eIF2alpha	GP	mutation of 	impair			near Ser51		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3063_s_290	15798194	(B and C) Mutations of eIF2alpha residues near and remote from Ser51 impair binding of eIF2B subunits to phosphorylated  eIF2alpha.	bind
10935	3	3499	7	11	NULL	0	NULL	eIF2alpha	GP	mutations of	impair			remote from Ser51		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3063_s_290	15798194	(B and C) Mutations of eIF2alpha residues near and remote from Ser51 impair binding of eIF2B subunits to phosphorylated  eIF2alpha.	bind
80744	1	3499	11	NULL	NULL	0	NULL	eIF2B	Protein		binds to 					eIF2alpha	Protein	phosphorylated			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_8_3063_s_290	15798194	(B and C) Mutations of eIF2alpha residues near and remote from Ser51 impair binding of eIF2B subunits to phosphorylated  eIF2alpha.	bind
80745	2	3499	11	NULL	NULL	0	NULL	eIF2alpha	Protein	mutation of	impair			near Ser51		statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_8_3063_s_290	15798194	(B and C) Mutations of eIF2alpha residues near and remote from Ser51 impair binding of eIF2B subunits to phosphorylated  eIF2alpha.	bind
80746	3	3499	11	NULL	NULL	0	NULL	eIF2alpha	Protein	mutation of	impair			remote from Ser51		statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_8_3063_s_290	15798194	(B and C) Mutations of eIF2alpha residues near and remote from Ser51 impair binding of eIF2B subunits to phosphorylated  eIF2alpha.	bind
7830	1	3500	6	11	NULL	0	NULL	Abl	GP	Purified;; recombinant;; Drosophila	bind					GST-Dlar	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_neuron_22_2_301_s_85	10069336	(B and C) Purified, recombinant  Drosophila Abl (B) or v-Abl (C) binds to GST-Dlar in vitro, as assessed by a pull down assay in which dAbl protein has been prelabeled with  32P-ATP before mixing with the fusion proteins.	bind
7831	2	3500	6	11	NULL	0	NULL	v-Abl	GP	Purified;; recombinant;; Drosophila	bind					GST-Dlar	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_neuron_22_2_301_s_85	10069336	(B and C) Purified, recombinant  Drosophila Abl (B) or v-Abl (C) binds to GST-Dlar in vitro, as assessed by a pull down assay in which dAbl protein has been prelabeled with  32P-ATP before mixing with the fusion proteins.	bind
10936	1	3500	7	11	NULL	0	NULL	Abl	GP	Purified;; recombinant;; Drosophila	binds					 GST-Dlar	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_neuron_22_2_301_s_85	10069336	(B and C) Purified, recombinant  Drosophila Abl (B) or v-Abl (C) binds to GST-Dlar in vitro, as assessed by a pull down assay in which dAbl protein has been prelabeled with  32P-ATP before mixing with the fusion proteins.	bind
10937	2	3500	7	11	NULL	0	NULL	v-Abl	GP	Purified;; recombinant;; Drosophila	binds					GST-Dlar	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_neuron_22_2_301_s_85	10069336	(B and C) Purified, recombinant  Drosophila Abl (B) or v-Abl (C) binds to GST-Dlar in vitro, as assessed by a pull down assay in which dAbl protein has been prelabeled with  32P-ATP before mixing with the fusion proteins.	bind
80747	1	3500	11	NULL	NULL	0	NULL	Abl	GeneOrProtein	Purified;;recombinant;;Drosophila	binds to 					GST-Dlar	Protein				NULL	in vitro	0	NULL	NULL	NULL	gw60_neuron_22_2_301_s_85	10069336	(B and C) Purified, recombinant  Drosophila Abl (B) or v-Abl (C) binds to GST-Dlar in vitro, as assessed by a pull down assay in which dAbl protein has been prelabeled with  32P-ATP before mixing with the fusion proteins.	bind
80748	2	3500	11	NULL	NULL	0	NULL	v-Abl	Protein		binds to 					GST-Dlar	Protein				NULL	in vitro	0	NULL	NULL	NULL	gw60_neuron_22_2_301_s_85	10069336	(B and C) Purified, recombinant  Drosophila Abl (B) or v-Abl (C) binds to GST-Dlar in vitro, as assessed by a pull down assay in which dAbl protein has been prelabeled with  32P-ATP before mixing with the fusion proteins.	bind
80749	3	3500	11	NULL	NULL	0	NULL	dAbl protein	Protein		prelabeled with					32P-ATP	Chemical				NULL		0	NULL	NULL	NULL	gw60_neuron_22_2_301_s_85	10069336	(B and C) Purified, recombinant  Drosophila Abl (B) or v-Abl (C) binds to GST-Dlar in vitro, as assessed by a pull down assay in which dAbl protein has been prelabeled with  32P-ATP before mixing with the fusion proteins.	bind
7833	1	3501	6	11	NULL	0	NULL	EGaseA	GP	Soybean	bind					GIP1	GP	P. sojae			NULL		NULL	NULL	NULL	NULL	gw70_genetics_169_2_1009_s_173	15545660	(b and c) Soybean EGaseA (solvent accessible surface) bound to  P. sojae GIP1 (ribbon diagram).	bind
10938	1	3501	7	11	NULL	0	NULL	EGaseA	GP	Soybean	bind					GIP1	GP	P. sojae			NULL		NULL	NULL	NULL	NULL	gw70_genetics_169_2_1009_s_173	15545660	(b and c) Soybean EGaseA (solvent accessible surface) bound to  P. sojae GIP1 (ribbon diagram).	bind
80750	1	3501	11	NULL	NULL	0	NULL	EGaseA	Protein	Soybean	binds to 					GIP1	Protein	P. sojae			NULL		0	NULL	NULL	NULL	gw70_genetics_169_2_1009_s_173	15545660	(b and c) Soybean EGaseA (solvent accessible surface) bound to  P. sojae GIP1 (ribbon diagram).	bind
7835	1	3502	6	11	NULL	0	NULL	p97	GP		bind					RanBP2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_8_12_2379_s_179	9398662	(B and C) Titration of p97 binding to RanBP2 and p62, respectively.	bind
7836	2	3502	6	11	NULL	0	NULL	p97	GP		bind					p62	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_8_12_2379_s_179	9398662	(B and C) Titration of p97 binding to RanBP2 and p62, respectively.	bind
10939	1	3502	7	11	NULL	0	NULL	p97	GP		bind					RanBP2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_8_12_2379_s_179	9398662	(B and C) Titration of p97 binding to RanBP2 and p62, respectively.	bind
10940	2	3502	7	11	NULL	0	NULL	p97	GP		bind					p62	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_8_12_2379_s_179	9398662	(B and C) Titration of p97 binding to RanBP2 and p62, respectively.	bind
80751	1	3502	11	NULL	NULL	NULL	NULL	p97	Protein	Titration	binds to 					RanBP2	Protein				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_8_12_2379_s_179	9398662	(B and C) Titration of p97 binding to RanBP2 and p62, respectively.	bind
80752	2	3502	11	NULL	NULL	0	NULL	 p97 	Protein	Titration	binds to 					p62	Protein				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_8_12_2379_s_179	9398662	(B and C) Titration of p97 binding to RanBP2 and p62, respectively.	bind
7837	1	3503	6	11	NULL	0	NULL	BCP	GP		bind					GPDH	GP	L.mexicana			NULL		NULL	NULL	NULL	NULL	gw60_chembiol_9_11_1189_s_59	12445769	(B and C) Two alternative conformations (conformation A, green; conformation B, red) of BCP bound to  L. mexicana GPDH in a model-unbiased, sigmaA-weighted Fo-Fc map (B) contoured at 3.5   (light brown) and an anomalous difference Fourier map contoured at 4.5   (red) and (C) an anomalous difference Fourier map contoured at 5.5   (red).	bind
11009	1	3503	7	11	NULL	0	NULL	BCP	GP		bind					GPDH	GP	L. mexicana 			NULL		NULL	NULL	NULL	NULL	gw60_chembiol_9_11_1189_s_59	12445769	(B and C) Two alternative conformations (conformation A, green; conformation B, red) of BCP bound to  L. mexicana GPDH in a model-unbiased, sigmaA-weighted Fo-Fc map (B) contoured at 3.5   (light brown) and an anomalous difference Fourier map contoured at 4.5   (red) and (C) an anomalous difference Fourier map contoured at 5.5   (red).	bind
80753	1	3503	11	NULL	NULL	0	NULL	BCP	Chemical		binds to 					GPDH	Protein	L. mexicana			NULL		0	NULL	NULL	NULL	gw60_chembiol_9_11_1189_s_59	12445769	(B and C) Two alternative conformations (conformation A, green; conformation B, red) of BCP bound to  L. mexicana GPDH in a model-unbiased, sigmaA-weighted Fo-Fc map (B) contoured at 3.5   (light brown) and an anomalous difference Fourier map contoured at 4.5   (red) and (C) an anomalous difference Fourier map contoured at 5.5   (red).	bind
7839	1	3505	6	11	NULL	0	NULL	Aft1	GP		bind					MRS4	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_15_6760_s_280	16024809	(B and D) In vivo DNA  binding of Aft1 and Aft2 to the  MRS4 promoter.	bind
7841	2	3505	6	11	NULL	0	NULL	Aft2	GP		bind					MRS4	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_15_6760_s_280	16024809	(B and D) In vivo DNA  binding of Aft1 and Aft2 to the  MRS4 promoter.	bind
11012	1	3505	7	11	NULL	0	NULL	Aft1	GP		bind					MRS4	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_15_6760_s_280	16024809	(B and D) In vivo DNA  binding of Aft1 and Aft2 to the  MRS4 promoter.	bind
11014	2	3505	7	11	NULL	0	NULL	Aft2	GP		bind					MRS4	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_15_6760_s_280	16024809	(B and D) In vivo DNA  binding of Aft1 and Aft2 to the  MRS4 promoter.	bind
80754	1	3505	11	NULL	NULL	NULL	NULL	Aft1	Protein		binds to 					MRS4 promoter	NucleicAcidSubstance				NULL	In vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_15_6760_s_280	16024809	(B and D) In vivo DNA  binding of Aft1 and Aft2 to the  MRS4 promoter.	bind
80755	2	3505	11	NULL	NULL	0	NULL	Aft2	Protein		binds to 					MRS4 promoter	NucleicAcidSubstance				NULL	in vivo	0	NULL	NULL	NULL	gw70_molcellbiol_25_15_6760_s_280	16024809	(B and D) In vivo DNA  binding of Aft1 and Aft2 to the  MRS4 promoter.	bind
7842	1	3506	6	11	NULL	0	NULL	Aft1	GP		bind					SMF3	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_15_6760_s_256	16024809	(B and D) In vivo DNA  binding of Aft1 and Aft2 to the  SMF3 promoter.	bind
7843	2	3506	6	11	NULL	0	NULL	Aft2	GP		bind					SMF3	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_15_6760_s_256	16024809	(B and D) In vivo DNA  binding of Aft1 and Aft2 to the  SMF3 promoter.	bind
11028	1	3506	7	11	NULL	0	NULL	Aft1	GP		bind					SMF3	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_15_6760_s_256	16024809	(B and D) In vivo DNA  binding of Aft1 and Aft2 to the  SMF3 promoter.	bind
11029	2	3506	7	11	NULL	0	NULL	Aft2	GP		bind					SMF3	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_15_6760_s_256	16024809	(B and D) In vivo DNA  binding of Aft1 and Aft2 to the  SMF3 promoter.	bind
80756	1	3506	11	NULL	NULL	0	NULL	Aft1	Protein		binds to 					SMF3 promoter	NucleicAcidSubstance				NULL	in vivo	0	NULL	NULL	NULL	gw70_molcellbiol_25_15_6760_s_256	16024809	(B and D) In vivo DNA  binding of Aft1 and Aft2 to the  SMF3 promoter.	bind
80757	2	3506	11	NULL	NULL	0	NULL	Aft2	Protein		binds to 					SMF3 promoter	NucleicAcidSubstance				NULL	in vivo	0	NULL	NULL	NULL	gw70_molcellbiol_25_15_6760_s_256	16024809	(B and D) In vivo DNA  binding of Aft1 and Aft2 to the  SMF3 promoter.	bind
7844	1	3507	6	11	NULL	0	NULL	Aft1-HA	GP		bind					FET3	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_15_6760_s_198	16024809	(B and D) In vivo DNA  binding of Aft1-HA and Aft2-HA to the  FET3 promoter.	bind
7845	2	3507	6	11	NULL	0	NULL	Aft2-HA	GP		bind					FET3	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_15_6760_s_198	16024809	(B and D) In vivo DNA  binding of Aft1-HA and Aft2-HA to the  FET3 promoter.	bind
11015	1	3507	7	11	NULL	0	NULL	 Aft1-HA	GP		bind					FET3	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_15_6760_s_198	16024809	(B and D) In vivo DNA  binding of Aft1-HA and Aft2-HA to the  FET3 promoter.	bind
11016	2	3507	7	11	NULL	0	NULL	Aft2-HA	GP		bind					FET3	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_15_6760_s_198	16024809	(B and D) In vivo DNA  binding of Aft1-HA and Aft2-HA to the  FET3 promoter.	bind
80758	1	3507	11	NULL	NULL	0	NULL	Aft1-HA	Protein		binds to 					FET3 promoter	NucleicAcidSubstance				NULL	in vivo	0	NULL	NULL	NULL	gw70_molcellbiol_25_15_6760_s_198	16024809	(B and D) In vivo DNA  binding of Aft1-HA and Aft2-HA to the  FET3 promoter.	bind
80759	2	3507	11	NULL	NULL	0	NULL	Aft2-HA	Protein		binds to 					FET3 promoter	NucleicAcidSubstance				NULL	in vivo	0	NULL	NULL	NULL	gw70_molcellbiol_25_15_6760_s_198	16024809	(B and D) In vivo DNA  binding of Aft1-HA and Aft2-HA to the  FET3 promoter.	bind
7848	1	3508	6	11	NULL	0	NULL	Aft1-HA	GP		bind					FTR1	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_15_6760_s_228	16024809	(B and D) In vivo DNA  binding of Aft1-HA and Aft2-HA to the  FTR1 promoter.	bind
7849	2	3508	6	11	NULL	0	NULL	Aft2-HA	GP		bind					FTR1	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_15_6760_s_228	16024809	(B and D) In vivo DNA  binding of Aft1-HA and Aft2-HA to the  FTR1 promoter.	bind
11017	1	3508	7	11	NULL	0	NULL	Aft1-HA	GP		bind					FTR1	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_15_6760_s_228	16024809	(B and D) In vivo DNA  binding of Aft1-HA and Aft2-HA to the  FTR1 promoter.	bind
11019	2	3508	7	11	NULL	0	NULL	Aft2-HA	GP		bind					FTR1	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_15_6760_s_228	16024809	(B and D) In vivo DNA  binding of Aft1-HA and Aft2-HA to the  FTR1 promoter.	bind
80760	1	3508	11	NULL	NULL	0	NULL	Aft1-HA	Protein		binds to 					FTR1 promoter	NucleicAcidSubstance				NULL	in vivo	0	NULL	NULL	NULL	gw70_molcellbiol_25_15_6760_s_228	16024809	(B and D) In vivo DNA  binding of Aft1-HA and Aft2-HA to the  FTR1 promoter.	bind
80761	2	3508	11	NULL	NULL	0	NULL	Aft2-HA	Protein		binds to 					 FTR1 promoter	NucleicAcidSubstance				NULL	in vivo	0	NULL	NULL	NULL	gw70_molcellbiol_25_15_6760_s_228	16024809	(B and D) In vivo DNA  binding of Aft1-HA and Aft2-HA to the  FTR1 promoter.	bind
7850	1	3509	6	11	NULL	0	NULL	GM1	GP		bind					EtxB	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_71_3_1527_s_145	12595472	(B to D) Analysis of Trp-fluorescence upon GM1 binding by EtxB, EtxB(G33D), and EtxB(H57S) by fluorescence spectroscopy.	bind
7851	2	3509	6	11	NULL	0	NULL	GM1	GP		bind					EtxB	Chemical		G33D		NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_71_3_1527_s_145	12595472	(B to D) Analysis of Trp-fluorescence upon GM1 binding by EtxB, EtxB(G33D), and EtxB(H57S) by fluorescence spectroscopy.	bind
7852	3	3509	6	11	NULL	0	NULL	GM1	GP		bind					EtxB	Chemical		H57S		NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_71_3_1527_s_145	12595472	(B to D) Analysis of Trp-fluorescence upon GM1 binding by EtxB, EtxB(G33D), and EtxB(H57S) by fluorescence spectroscopy.	bind
11020	1	3509	7	11	NULL	0	NULL	GM1	GP		bind					EtxB	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_71_3_1527_s_145	12595472	(B to D) Analysis of Trp-fluorescence upon GM1 binding by EtxB, EtxB(G33D), and EtxB(H57S) by fluorescence spectroscopy.	bind
11021	2	3509	7	11	NULL	0	NULL	GM1	GP		bind					EtxB	Chemical		G33D		NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_71_3_1527_s_145	12595472	(B to D) Analysis of Trp-fluorescence upon GM1 binding by EtxB, EtxB(G33D), and EtxB(H57S) by fluorescence spectroscopy.	bind
11022	3	3509	7	11	NULL	0	NULL	GM1	GP		bind					EtxB	Chemical		H57S		NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_71_3_1527_s_145	12595472	(B to D) Analysis of Trp-fluorescence upon GM1 binding by EtxB, EtxB(G33D), and EtxB(H57S) by fluorescence spectroscopy.	bind
80762	1	3509	11	NULL	NULL	NULL	NULL	GM1	Protein		binds to 					EtxB	Protein				NULL	fluorescence spectroscopy	NULL	NULL	NULL	NULL	gw60_infectimmun_71_3_1527_s_145	12595472	(B to D) Analysis of Trp-fluorescence upon GM1 binding by EtxB, EtxB(G33D), and EtxB(H57S) by fluorescence spectroscopy.	bind
80763	2	3509	11	NULL	NULL	0	NULL	GM1	Protein		binds to 					EtxB(G33D)	Protein				NULL	fluorescence spectroscopy	0	NULL	NULL	NULL	gw60_infectimmun_71_3_1527_s_145	12595472	(B to D) Analysis of Trp-fluorescence upon GM1 binding by EtxB, EtxB(G33D), and EtxB(H57S) by fluorescence spectroscopy.	bind
80764	3	3509	11	NULL	NULL	0	NULL	GM1	Protein		binds to 					EtxB(H57S)	Protein				NULL	fluorescence spectroscopy	0	NULL	NULL	NULL	gw60_infectimmun_71_3_1527_s_145	12595472	(B to D) Analysis of Trp-fluorescence upon GM1 binding by EtxB, EtxB(G33D), and EtxB(H57S) by fluorescence spectroscopy.	bind
7853	1	3510	6	11	NULL	0	NULL	AML family 	GP		bind					NP-3	GP			promoter sequences	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_322_s_101	9418879	(B to D) Binding of AML family members to NP-3 promoter sequences determined by electrophoretic mobility shift assays.	bind
11025	1	3510	7	11	NULL	0	NULL	AML family	GP		bind					NP-3	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_322_s_101	9418879	(B to D) Binding of AML family members to NP-3 promoter sequences determined by electrophoretic mobility shift assays.	bind
81257	2	3510	11	NULL	NULL	0	NULL	AML family members	Protein		binds to 					NP-3	Gene			promoter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_322_s_101	9418879	(B to D) Binding of AML family members to NP-3 promoter sequences determined by electrophoretic mobility shift assays.	bind
7854	1	3513	6	11	NULL	0	NULL	ASH1	GP	transcription of	is dependent on					Swi5p	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_84_5_699_s_141	8625408	(B)  ASH1 transcription is dependent on Swi5p and Ace2p transcription  factors.	bind
7855	2	3513	6	11	NULL	0	NULL	ASH1	GP	transcription of	is dependent on					Ace2p	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_84_5_699_s_141	8625408	(B)  ASH1 transcription is dependent on Swi5p and Ace2p transcription  factors.	bind
11089	1	3513	7	11	NULL	0	NULL	ASH1	GP	transcription of	is dependent on					Swi5p	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_84_5_699_s_141	8625408	(B)  ASH1 transcription is dependent on Swi5p and Ace2p transcription  factors.	bind
11090	2	3513	7	11	NULL	0	NULL	ASH1	GP	transcription of	is dependent on					Ace2p	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_84_5_699_s_141	8625408	(B)  ASH1 transcription is dependent on Swi5p and Ace2p transcription  factors.	bind
80766	1	3513	11	NULL	NULL	0	NULL	ASH1	Gene		undergoes					transcription	MolecularProcess				NULL		0	NULL	NULL	NULL	gw60_cell_84_5_699_s_141	8625408	(B)  ASH1 transcription is dependent on Swi5p and Ace2p transcription  factors.	bind
80767	2	3513	11	NULL	NULL	0	NULL	statement 1	Process		depends on					Swi5p transcription factor	Protein				NULL		0	NULL	NULL	NULL	gw60_cell_84_5_699_s_141	8625408	(B)  ASH1 transcription is dependent on Swi5p and Ace2p transcription  factors.	bind
80768	3	3513	11	NULL	NULL	NULL	NULL	statement 1	Process		depends on					Ace2p transcription factor	Protein				NULL		NULL	NULL	NULL	NULL	gw60_cell_84_5_699_s_141	8625408	(B)  ASH1 transcription is dependent on Swi5p and Ace2p transcription  factors.	bind
7856	1	3515	6	11	NULL	NULL	NULL	bacteria	Organism		bind					NK cells	Cell	purified;; human			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_74_7_4133_s_156	16790787	(B)  Binding of bacteria to purified NK cells from two different human donors.	bind
11092	1	3515	7	11	NULL	NULL	NULL	bacteria	Organism		bind					NK cells	Cell	human;; purified			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_74_7_4133_s_156	16790787	(B)  Binding of bacteria to purified NK cells from two different human donors.	bind
80769	1	3515	11	NULL	NULL	0	NULL	 NK cells	cell	purified;;from human donor	binds to 					bacteria	Organism				NULL		0	NULL	NULL	NULL	gw70_infectimmun_74_7_4133_s_156	16790787	(B)  Binding of bacteria to purified NK cells from two different human donors.	bind
11093	1	3516	7	11	NULL	NULL	NULL	Smurf1	GP		bind			CA		Smad5	GP	WT			NULL	transfected COS7 cells	NULL	NULL	NULL	NULL	gw60_molbiolcell_14_7_2809_s_105	12857866	(B)  Binding of Smurf1(CA) to Smad5(WT) and Smad5(deltaPY) was examined in  transfected COS7 cells.	bind
11094	2	3516	7	11	NULL	NULL	NULL	Smurf1	GP		bind			CA		Smad5	GP		deltaPY		NULL	transfected COS7 cells	NULL	NULL	NULL	NULL	gw60_molbiolcell_14_7_2809_s_105	12857866	(B)  Binding of Smurf1(CA) to Smad5(WT) and Smad5(deltaPY) was examined in  transfected COS7 cells.	bind
80770	1	3516	11	NULL	NULL	0	NULL	Smurf1(CA)	Protein		binds to 					Smad5(WT)					NULL	transfected COS7 cells	0	NULL	NULL	NULL	gw60_molbiolcell_14_7_2809_s_105	12857866	(B)  Binding of Smurf1(CA) to Smad5(WT) and Smad5(deltaPY) was examined in  transfected COS7 cells.	bind
80771	2	3516	11	NULL	NULL	0	NULL	Smurf1(CA)	Protein		binds to 					Smad5(deltaPY)	Protein				NULL	transfected COS7 cells	0	NULL	NULL	NULL	gw60_molbiolcell_14_7_2809_s_105	12857866	(B)  Binding of Smurf1(CA) to Smad5(WT) and Smad5(deltaPY) was examined in  transfected COS7 cells.	bind
7878	1	3518	6	11	NULL	NULL	NULL	myoB	GP	Dictyostelium	bind			SH3 domain		p116	GP		proline-rich motifs		NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1525_3_245_s_212	11257438	(B)  Dictyostelium myoB and myoC bind via their SH3 domain to proline-rich motifs within p116, a scaffold protein that also binds capping protein (CP) and the Arp2/3 complex.	bind
7885	2	3518	6	11	NULL	NULL	NULL	myoC	GP	Dictyostelium	bind			SH3 domain		p116	GP		proline-rich motifs		NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1525_3_245_s_212	11257438	(B)  Dictyostelium myoB and myoC bind via their SH3 domain to proline-rich motifs within p116, a scaffold protein that also binds capping protein (CP) and the Arp2/3 complex.	bind
7886	3	3518	6	11	NULL	NULL	NULL	p116	GP		bind					CP	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1525_3_245_s_212	11257438	(B)  Dictyostelium myoB and myoC bind via their SH3 domain to proline-rich motifs within p116, a scaffold protein that also binds capping protein (CP) and the Arp2/3 complex.	bind
7887	4	3518	6	11	NULL	NULL	NULL	p116	GP		bind					Arp2/3 complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1525_3_245_s_212	11257438	(B)  Dictyostelium myoB and myoC bind via their SH3 domain to proline-rich motifs within p116, a scaffold protein that also binds capping protein (CP) and the Arp2/3 complex.	bind
40771	5	3518	6	11	NULL	NULL	NULL	p116	GP		is a type of					scaffold protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1525_3_245_s_212	11257438	(B)  Dictyostelium myoB and myoC bind via their SH3 domain to proline-rich motifs within p116, a scaffold protein that also binds capping protein (CP) and the Arp2/3 complex.	bind
40772	6	3518	6	11	NULL	NULL	NULL	CP	GP		is					capping protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1525_3_245_s_212	11257438	(B)  Dictyostelium myoB and myoC bind via their SH3 domain to proline-rich motifs within p116, a scaffold protein that also binds capping protein (CP) and the Arp2/3 complex.	bind
11095	1	3518	7	11	NULL	NULL	NULL	myoB	GP	Dictyostelium	bind			SH3 domain		p116	GP		proline-rich motifs		NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1525_3_245_s_212	11257438	(B)  Dictyostelium myoB and myoC bind via their SH3 domain to proline-rich motifs within p116, a scaffold protein that also binds capping protein (CP) and the Arp2/3 complex.	bind
11096	2	3518	7	11	NULL	NULL	NULL	myoC	GP	Dictyostelium	bind			SH3 domain		p116	GP		 proline-rich motifs		NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1525_3_245_s_212	11257438	(B)  Dictyostelium myoB and myoC bind via their SH3 domain to proline-rich motifs within p116, a scaffold protein that also binds capping protein (CP) and the Arp2/3 complex.	bind
11099	3	3518	7	11	NULL	NULL	NULL	p116	GP		bind					capping protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1525_3_245_s_212	11257438	(B)  Dictyostelium myoB and myoC bind via their SH3 domain to proline-rich motifs within p116, a scaffold protein that also binds capping protein (CP) and the Arp2/3 complex.	bind
11100	4	3518	7	11	NULL	NULL	NULL	p116	GP		bind					Arp2/3 complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1525_3_245_s_212	11257438	(B)  Dictyostelium myoB and myoC bind via their SH3 domain to proline-rich motifs within p116, a scaffold protein that also binds capping protein (CP) and the Arp2/3 complex.	bind
11102	5	3518	7	11	NULL	NULL	NULL	p116	GP		is a type of					scaffold protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1525_3_245_s_212	11257438	(B)  Dictyostelium myoB and myoC bind via their SH3 domain to proline-rich motifs within p116, a scaffold protein that also binds capping protein (CP) and the Arp2/3 complex.	bind
11104	6	3518	7	11	NULL	NULL	NULL	capping protein	GP		is					CP	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1525_3_245_s_212	11257438	(B)  Dictyostelium myoB and myoC bind via their SH3 domain to proline-rich motifs within p116, a scaffold protein that also binds capping protein (CP) and the Arp2/3 complex.	bind
80772	1	3518	11	NULL	NULL	0	NULL	p116	Protein		is a type of 					scaffold protein	Protein				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1525_3_245_s_212	11257438	(B)  Dictyostelium myoB and myoC bind via their SH3 domain to proline-rich motifs within p116, a scaffold protein that also binds capping protein (CP) and the Arp2/3 complex.	bind
80773	2	3518	11	NULL	NULL	0	NULL	p116	Protein		binds to 					capping protein	Protein				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1525_3_245_s_212	11257438	(B)  Dictyostelium myoB and myoC bind via their SH3 domain to proline-rich motifs within p116, a scaffold protein that also binds capping protein (CP) and the Arp2/3 complex.	bind
80774	3	3518	11	NULL	NULL	0	NULL	p116	Protein		binds to 					Arp2/3 complex	Protein				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1525_3_245_s_212	11257438	(B)  Dictyostelium myoB and myoC bind via their SH3 domain to proline-rich motifs within p116, a scaffold protein that also binds capping protein (CP) and the Arp2/3 complex.	bind
80775	4	3518	11	NULL	NULL	0	NULL	capping protein	Protein		is					CP	Protein				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1525_3_245_s_212	11257438	(B)  Dictyostelium myoB and myoC bind via their SH3 domain to proline-rich motifs within p116, a scaffold protein that also binds capping protein (CP) and the Arp2/3 complex.	bind
80776	5	3518	11	NULL	NULL	0	NULL	myoB	Protein	Dictyostelium	binds to 			SH3 domain		p116	Protein		proline-rich motifs		NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1525_3_245_s_212	11257438	(B)  Dictyostelium myoB and myoC bind via their SH3 domain to proline-rich motifs within p116, a scaffold protein that also binds capping protein (CP) and the Arp2/3 complex.	bind
80777	6	3518	11	NULL	NULL	0	NULL	myoC	Protein	Dictyostelium	binds to 			SH3 domain		p116	Protein		proline-rich motif		NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1525_3_245_s_212	11257438	(B)  Dictyostelium myoB and myoC bind via their SH3 domain to proline-rich motifs within p116, a scaffold protein that also binds capping protein (CP) and the Arp2/3 complex.	bind
7964	1	3519	6	11	NULL	NULL	NULL	Wsp	GP	Drosophila	bind					CDC42	GP	activated			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_1_1_s_87	11149916	(B)  Drosophila Wsp binds the activated form of CDC42 in a blot overlay assay.	bind
11106	1	3519	7	11	NULL	NULL	NULL	Wsp	GP	Drosophila	bind					CDC42	GP	activated			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_1_1_s_87	11149916	(B)  Drosophila Wsp binds the activated form of CDC42 in a blot overlay assay.	bind
80778	1	3519	11	NULL	NULL	0	NULL	Wsp	Protein	Drosophila	binds to 					CDC42	Protein	activated			NULL	blot overlay assay	0	NULL	NULL	NULL	gw60_cellbiol_152_1_1_s_87	11149916	(B)  Drosophila Wsp binds the activated form of CDC42 in a blot overlay assay.	bind
7965	1	3520	6	11	NULL	NULL	NULL	Smad7	GP	endogenous	bind					p38	GP	phosphorylated			NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molbiolcell_14_2_529_s_245	12589052	(B)  Endogenous Smad7 binds to phosphorylated p38 in vivo.	bind
11111	1	3520	7	11	NULL	NULL	NULL	Smad7	GP	endogenous	bind					p38	GP	phosphorylated			NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molbiolcell_14_2_529_s_245	12589052	(B)  Endogenous Smad7 binds to phosphorylated p38 in vivo.	bind
80779	1	3520	11	NULL	NULL	0	NULL	Smad7	Protein	Endogenous	binds to 					p38	Protein	phosphorylated			NULL	in vivo	0	NULL	NULL	NULL	gw70_molbiolcell_14_2_529_s_245	12589052	(B)  Endogenous Smad7 binds to phosphorylated p38 in vivo.	bind
7966	1	3521	6	11	NULL	NULL	NULL	GST-Mst27p-AAXX	GP		does not bind					coatomer	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_8_3097_s_242	12925749	(B)  GST-Mst27p-AAXX and GST-Prm8p do not bind to coatomer.	bind
7967	2	3521	6	11	NULL	NULL	NULL	GST-Prm8p	GP		does not bind					coatomer	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_8_3097_s_242	12925749	(B)  GST-Mst27p-AAXX and GST-Prm8p do not bind to coatomer.	bind
11113	1	3521	7	11	NULL	NULL	NULL	GST-Mst27p-AAXX	GP		does not bind					coatomer	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_8_3097_s_242	12925749	(B)  GST-Mst27p-AAXX and GST-Prm8p do not bind to coatomer.	bind
11115	2	3521	7	11	NULL	NULL	NULL	GST-Prm8p	GP		does not bind					coatomer	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_8_3097_s_242	12925749	(B)  GST-Mst27p-AAXX and GST-Prm8p do not bind to coatomer.	bind
80780	1	3521	11	NULL	NULL	0	NULL	GST-Mst27p-AAXX	Protein		does not bind to					coatomer	Protein				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_8_3097_s_242	12925749	(B)  GST-Mst27p-AAXX and GST-Prm8p do not bind to coatomer.	bind
80781	2	3521	11	NULL	NULL	0	NULL	GST-Prm8p	Protein		does not bind to					coatomer	Protein				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_8_3097_s_242	12925749	(B)  GST-Mst27p-AAXX and GST-Prm8p do not bind to coatomer.	bind
7968	1	3522	6	11	NULL	NULL	NULL	Stat1	GP		bind					DNA	NucleicAcid				NULL	HEp-2 cells	NULL	NULL	NULL	NULL	gw70_infectimmun_72_1_537_s_154	14688135	(B)  HEp-2 cells demonstrated inducible STAT1 DNA binding in response to stimulation with  IFN-gamma (20 ng/ml, 30 min) (arrow, lane 2).	bind
8174	2	3522	6	11	NULL	NULL	NULL	IFN-gamma	GP		induces					statement 1	Process				NULL	HEp-2 cells	NULL	NULL	NULL	NULL	gw70_infectimmun_72_1_537_s_154	14688135	(B)  HEp-2 cells demonstrated inducible STAT1 DNA binding in response to stimulation with  IFN-gamma (20 ng/ml, 30 min) (arrow, lane 2).	bind
11118	1	3522	7	11	NULL	NULL	NULL	STAT1	GP		bind					DNA	NucleicAcid				NULL	HEp-2 cells	NULL	NULL	NULL	NULL	gw70_infectimmun_72_1_537_s_154	14688135	(B)  HEp-2 cells demonstrated inducible STAT1 DNA binding in response to stimulation with  IFN-gamma (20 ng/ml, 30 min) (arrow, lane 2).	bind
11120	2	3522	7	11	NULL	NULL	NULL	HEp-2 cells	Cell		stimulated with					IFN-gamma	GP				NULL	HEp-2 cells	NULL	NULL	NULL	NULL	gw70_infectimmun_72_1_537_s_154	14688135	(B)  HEp-2 cells demonstrated inducible STAT1 DNA binding in response to stimulation with  IFN-gamma (20 ng/ml, 30 min) (arrow, lane 2).	bind
11121	3	3522	7	11	NULL	NULL	NULL	statement 2	Process		induce					statement 1	Process				NULL	HEp-2 cells	NULL	NULL	NULL	NULL	gw70_infectimmun_72_1_537_s_154	14688135	(B)  HEp-2 cells demonstrated inducible STAT1 DNA binding in response to stimulation with  IFN-gamma (20 ng/ml, 30 min) (arrow, lane 2).	bind
80782	1	3522	11	NULL	NULL	0	NULL	STAT1	Protein		binds to 					DNA	NucleicAcidSubstance				NULL	HEp-2 cells	0	NULL	NULL	NULL	gw70_infectimmun_72_1_537_s_154	14688135	(B)  HEp-2 cells demonstrated inducible STAT1 DNA binding in response to stimulation with  IFN-gamma (20 ng/ml, 30 min) (arrow, lane 2).	bind
80783	2	3522	11	NULL	NULL	0	NULL	IFN-gamma	Protein		stimulates					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_infectimmun_72_1_537_s_154	14688135	(B)  HEp-2 cells demonstrated inducible STAT1 DNA binding in response to stimulation with  IFN-gamma (20 ng/ml, 30 min) (arrow, lane 2).	bind
7969	1	3523	6	11	NULL	NULL	NULL	GFP-coronin	GP		bind					F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_4_1275_s_130	10749929	(B)  limB null and KAx-3 cells expressing GFP-coronin, which binds to F-actin.	bind
7970	2	3523	6	11	NULL	NULL	NULL	limB null cells	Cell		express					GFP-coronin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_4_1275_s_130	10749929	(B)  limB null and KAx-3 cells expressing GFP-coronin, which binds to F-actin.	bind
7971	3	3523	6	11	NULL	NULL	NULL	KAx-3 cells	Cell		express					GFP-coronin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_4_1275_s_130	10749929	(B)  limB null and KAx-3 cells expressing GFP-coronin, which binds to F-actin.	bind
11124	1	3523	7	11	NULL	NULL	NULL	limB null cells	Cell		express					GFP-coronin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_4_1275_s_130	10749929	(B)  limB null and KAx-3 cells expressing GFP-coronin, which binds to F-actin.	bind
11126	2	3523	7	11	NULL	NULL	NULL	KAx-3 cells	Cell	 	express					GFP-coronin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_4_1275_s_130	10749929	(B)  limB null and KAx-3 cells expressing GFP-coronin, which binds to F-actin.	bind
15046	3	3523	7	11	NULL	NULL	NULL	GFP-coronin	GP		binds					F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_4_1275_s_130	10749929	(B)  limB null and KAx-3 cells expressing GFP-coronin, which binds to F-actin.	bind
80784	1	3523	11	NULL	NULL	0	NULL	GFP-coronin	Protein		binds to 					F-actin	Protein				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1275_s_130	10749929	(B)  limB null and KAx-3 cells expressing GFP-coronin, which binds to F-actin.	bind
80785	2	3523	11	NULL	NULL	0	NULL	limB null cells	cell		express					GFP-coronin	Protein				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1275_s_130	10749929	(B)  limB null and KAx-3 cells expressing GFP-coronin, which binds to F-actin.	bind
80786	3	3523	11	NULL	NULL	0	NULL	KAx-3 cell	cell		express					GFP-coronin	Protein				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1275_s_130	10749929	(B)  limB null and KAx-3 cells expressing GFP-coronin, which binds to F-actin.	bind
7972	1	3524	6	11	NULL	NULL	NULL	M. tuberculosis	Organism		bind					M cell surface	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_immunity_10_6_641_s_64	10403639	(B)  M. tuberculosis (arrowheads) binds to the M cell surface and is internalized.	bind
7973	2	3524	6	11	NULL	NULL	NULL	statement 1	Process		leads to					M. tuberculosis	Organism	internalization of			NULL		NULL	NULL	NULL	NULL	gw60_immunity_10_6_641_s_64	10403639	(B)  M. tuberculosis (arrowheads) binds to the M cell surface and is internalized.	bind
11127	1	3524	7	11	NULL	NULL	NULL	M. tuberculosis	Organism		bind					M cell surface	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_immunity_10_6_641_s_64	10403639	(B)  M. tuberculosis (arrowheads) binds to the M cell surface and is internalized.	bind
11128	2	3524	7	11	NULL	NULL	NULL	statement 1	Process		leads to 					M. tuberculosis	Organism	internalization of			NULL		NULL	NULL	NULL	NULL	gw60_immunity_10_6_641_s_64	10403639	(B)  M. tuberculosis (arrowheads) binds to the M cell surface and is internalized.	bind
80787	1	3524	11	NULL	NULL	0	NULL	M. tuberculosis	Organism		binds to 					M cell 	Cell	surface			NULL		0	NULL	NULL	NULL	gw60_immunity_10_6_641_s_64	10403639	(B)  M. tuberculosis (arrowheads) binds to the M cell surface and is internalized.	bind
80788	2	3524	11	NULL	NULL	0	NULL	statement 1	Process		leads to					internalization 	BiologicalProcess	M cell			NULL		0	NULL	NULL	NULL	gw60_immunity_10_6_641_s_64	10403639	(B)  M. tuberculosis (arrowheads) binds to the M cell surface and is internalized.	bind
7974	1	3526	6	11	NULL	NULL	NULL	A-Myb	GP		bind					GST-CBP	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4705_s_195	16055500	(B)  NLK blocks the binding of A-Myb to GST-CBP.	bind
7975	2	3526	6	11	NULL	NULL	NULL	NLK	GP		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4705_s_195	16055500	(B)  NLK blocks the binding of A-Myb to GST-CBP.	bind
11130	1	3526	7	11	NULL	NULL	NULL	A-Myb	GP		binds					GST-CBP	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4705_s_195	16055500	(B)  NLK blocks the binding of A-Myb to GST-CBP.	bind
11132	2	3526	7	11	NULL	NULL	NULL	 NLK	GP		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4705_s_195	16055500	(B)  NLK blocks the binding of A-Myb to GST-CBP.	bind
80789	1	3526	11	NULL	NULL	0	NULL	A-Myb	Protein		binds to 					GST-CBP	Protein				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4705_s_195	16055500	(B)  NLK blocks the binding of A-Myb to GST-CBP.	bind
80790	2	3526	11	NULL	NULL	0	NULL	NLK	Protein		blocks					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4705_s_195	16055500	(B)  NLK blocks the binding of A-Myb to GST-CBP.	bind
7976	1	3527	6	11	NULL	NULL	NULL	PAX	GP		bind					PIX	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_4_851_s_265	10330411	(B)  PAK bound to PIX as previously reported.	bind
11133	1	3527	7	11	NULL	NULL	NULL	PAK 	GP		bind					PIX	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_4_851_s_265	10330411	(B)  PAK bound to PIX as previously reported.	bind
80791	1	3527	11	NULL	NULL	0	NULL	PAK	Protein		binds to 					 PIX	Protein				NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_4_851_s_265	10330411	(B)  PAK bound to PIX as previously reported.	bind
7977	1	3528	6	11	NULL	NULL	NULL	Stat3	GP		bind					p53	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_17_7432_s_160	16107692	(B)  PDGF stimulation (10 ng/ml for 8 h), which activates Stat3, also leads to Stat3 binding  to the p53 promoter region as shown by ChIP.	bind
7978	2	3528	6	11	NULL	NULL	NULL	PDGF	GP	stimulation of	leads to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_17_7432_s_160	16107692	(B)  PDGF stimulation (10 ng/ml for 8 h), which activates Stat3, also leads to Stat3 binding  to the p53 promoter region as shown by ChIP.	bind
7979	3	3528	6	11	NULL	NULL	NULL	PDGF	GP	stimulation of	activates					Stat3	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_17_7432_s_160	16107692	(B)  PDGF stimulation (10 ng/ml for 8 h), which activates Stat3, also leads to Stat3 binding  to the p53 promoter region as shown by ChIP.	bind
11165	1	3528	7	11	NULL	NULL	NULL	Stat3 	GP		bind					p53	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_17_7432_s_160	16107692	(B)  PDGF stimulation (10 ng/ml for 8 h), which activates Stat3, also leads to Stat3 binding  to the p53 promoter region as shown by ChIP.	bind
11166	2	3528	7	11	NULL	NULL	NULL	PDGF	GP	stimulation of	activates					Stat3	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_17_7432_s_160	16107692	(B)  PDGF stimulation (10 ng/ml for 8 h), which activates Stat3, also leads to Stat3 binding  to the p53 promoter region as shown by ChIP.	bind
11167	3	3528	7	11	NULL	NULL	NULL	PDGF	GP	stimulation of	activates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_17_7432_s_160	16107692	(B)  PDGF stimulation (10 ng/ml for 8 h), which activates Stat3, also leads to Stat3 binding  to the p53 promoter region as shown by ChIP.	bind
80792	1	3528	11	NULL	NULL	NULL	NULL	Stat3	Protein		binds to 					p53 promoter	NucleicAcidSubstance				NULL	ChIP	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_17_7432_s_160	16107692	(B)  PDGF stimulation (10 ng/ml for 8 h), which activates Stat3, also leads to Stat3 binding  to the p53 promoter region as shown by ChIP.	bind
80793	2	3528	11	NULL	NULL	0	NULL	PDGF	Protein	active	activates					Stat3	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_17_7432_s_160	16107692	(B)  PDGF stimulation (10 ng/ml for 8 h), which activates Stat3, also leads to Stat3 binding  to the p53 promoter region as shown by ChIP.	bind
80794	3	3528	11	NULL	NULL	0	NULL	statement 2	Process		leads to					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_17_7432_s_160	16107692	(B)  PDGF stimulation (10 ng/ml for 8 h), which activates Stat3, also leads to Stat3 binding  to the p53 promoter region as shown by ChIP.	bind
7980	1	3530	6	11	NULL	NULL	NULL	TFIID	GP	S. cerevisiae	bind		specifically			Ad2 MLP	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_16_6000_s_163	12138208	(B)  S. cerevisiae TFIID binds the Ad2 MLP specifically.	bind
11168	1	3530	7	11	NULL	NULL	NULL	TFIID	GP	S. cerevisiae	binds		specifically			Ad2 MLP 	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_16_6000_s_163	12138208	(B)  S. cerevisiae TFIID binds the Ad2 MLP specifically.	bind
80795	1	3530	11	NULL	NULL	0	NULL	TFIID	Protein	S. cerevisiae	binds to 		specifically			Ad2 MLP	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_16_6000_s_163	12138208	(B)  S. cerevisiae TFIID binds the Ad2 MLP specifically.	bind
7981	1	3532	6	11	NULL	NULL	NULL	RANTES	GP	125I-labeled	bind					CHO-CCR5 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_151_6_1281_s_184	11121442	(B) 125I-RANTES (closed symbols) and 125I - AOP-RANTES (open symbols) were bound to CHO-CCR5 (  and  ) or CHO-K1 (.,  ) cells as described in A.	bind
7982	2	3532	6	11	NULL	NULL	NULL	RANTES	GP	125I-labeled	bind					CHO-K1 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_151_6_1281_s_184	11121442	(B) 125I-RANTES (closed symbols) and 125I - AOP-RANTES (open symbols) were bound to CHO-CCR5 (  and  ) or CHO-K1 (.,  ) cells as described in A.	bind
7983	3	3532	6	11	NULL	NULL	NULL	AOP-RANTES	GP	125I-labeled	bind					CHO-CCR5 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_151_6_1281_s_184	11121442	(B) 125I-RANTES (closed symbols) and 125I - AOP-RANTES (open symbols) were bound to CHO-CCR5 (  and  ) or CHO-K1 (.,  ) cells as described in A.	bind
7984	4	3532	6	11	NULL	NULL	NULL	AOP-RANTES	GP	125I-labeled	bind					CHO-K1 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_151_6_1281_s_184	11121442	(B) 125I-RANTES (closed symbols) and 125I - AOP-RANTES (open symbols) were bound to CHO-CCR5 (  and  ) or CHO-K1 (.,  ) cells as described in A.	bind
11169	1	3532	7	11	NULL	NULL	NULL	RANTES	GP	125I-labeled	bind					CHO-CCR5 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_151_6_1281_s_184	11121442	(B) 125I-RANTES (closed symbols) and 125I - AOP-RANTES (open symbols) were bound to CHO-CCR5 (  and  ) or CHO-K1 (.,  ) cells as described in A.	bind
11170	2	3532	7	11	NULL	NULL	NULL	RANTES	GP	125I-labeled	bind					CHO-K1 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_151_6_1281_s_184	11121442	(B) 125I-RANTES (closed symbols) and 125I - AOP-RANTES (open symbols) were bound to CHO-CCR5 (  and  ) or CHO-K1 (.,  ) cells as described in A.	bind
11171	3	3532	7	11	NULL	NULL	NULL	AOP-RANTES	GP	125I-labeled	bind					CHO-CCR5 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_151_6_1281_s_184	11121442	(B) 125I-RANTES (closed symbols) and 125I - AOP-RANTES (open symbols) were bound to CHO-CCR5 (  and  ) or CHO-K1 (.,  ) cells as described in A.	bind
11172	4	3532	7	11	NULL	NULL	NULL	AOP-RANTES	GP	125I-labeled	bind					CHO-K1 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_151_6_1281_s_184	11121442	(B) 125I-RANTES (closed symbols) and 125I - AOP-RANTES (open symbols) were bound to CHO-CCR5 (  and  ) or CHO-K1 (.,  ) cells as described in A.	bind
80796	1	3532	11	NULL	NULL	0	NULL	125I-RANTES	Protein		binds to 					CHO-CCR5 cells	Cell				NULL		0	NULL	NULL	NULL	gw60_cellbiol_151_6_1281_s_184	11121442	(B) 125I-RANTES (closed symbols) and 125I - AOP-RANTES (open symbols) were bound to CHO-CCR5 (  and  ) or CHO-K1 (.,  ) cells as described in A.	bind
80797	2	3532	11	NULL	NULL	0	NULL	125I-RANTES	Protein		binds to 					CHO-K1 cell	Cell				NULL		0	NULL	NULL	NULL	gw60_cellbiol_151_6_1281_s_184	11121442	(B) 125I-RANTES (closed symbols) and 125I - AOP-RANTES (open symbols) were bound to CHO-CCR5 (  and  ) or CHO-K1 (.,  ) cells as described in A.	bind
80798	3	3532	11	NULL	NULL	0	NULL	125I - AOP-RANTES	Protein		binds to 					CHO-CCR5 cells	Cell				NULL		0	NULL	NULL	NULL	gw60_cellbiol_151_6_1281_s_184	11121442	(B) 125I-RANTES (closed symbols) and 125I - AOP-RANTES (open symbols) were bound to CHO-CCR5 (  and  ) or CHO-K1 (.,  ) cells as described in A.	bind
80799	4	3532	11	NULL	NULL	0	NULL	125I - AOP-RANTES	Protein		binds to 					CHO-K1 cell	Cell				NULL		0	NULL	NULL	NULL	gw60_cellbiol_151_6_1281_s_184	11121442	(B) 125I-RANTES (closed symbols) and 125I - AOP-RANTES (open symbols) were bound to CHO-CCR5 (  and  ) or CHO-K1 (.,  ) cells as described in A.	bind
7985	1	3537	6	11	NULL	NULL	NULL	SEP-1 protein	GP	35S-labeled	bind					GST-IFY-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_24_2118_s_145	12498686	(b) 35S-labeled SEP-1 protein binds GST-IFY-1.	bind
11173	1	3537	7	11	NULL	NULL	NULL	 SEP-1 protein	GP	35S-labeled	binds					GST-IFY-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_24_2118_s_145	12498686	(b) 35S-labeled SEP-1 protein binds GST-IFY-1.	bind
80800	1	3537	11	NULL	NULL	0	NULL	SEP-1 protein	Protein	35S-labeled	binds to 					GST-IFY-1	Protein				NULL		0	NULL	NULL	NULL	gw60_currbiol_12_24_2118_s_145	12498686	(b) 35S-labeled SEP-1 protein binds GST-IFY-1.	bind
7986	1	3539	6	11	NULL	NULL	NULL	SR protein	GP		bind									exon N1	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_6_1874_s_155	12612063	(B) A 35-kDa SR protein binds to exon N1.	bind
11174	1	3539	7	11	NULL	NULL	NULL	SR protein	GP		binds to									exon N1	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_6_1874_s_155	12612063	(B) A 35-kDa SR protein binds to exon N1.	bind
80801	1	3539	11	NULL	NULL	0	NULL	SR protein	Protein		binds to 					exon N1	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_6_1874_s_155	12612063	(B) A 35-kDa SR protein binds to exon N1.	bind
7987	1	3540	6	11	NULL	NULL	NULL	PlexB	GP		bind					RhoA	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_1_39_s_89	11604137	(B) A bigger region of PlexB, PlexB  also binds to RhoA.	bind
11175	1	3540	7	11	NULL	NULL	NULL	PlexB	GP		binds					RhoA	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_1_39_s_89	11604137	(B) A bigger region of PlexB, PlexB  also binds to RhoA.	bind
80802	1	3540	11	NULL	NULL	0	NULL	PlexB	Protein		binds to 					RhoA	Protein				NULL		0	NULL	NULL	NULL	gw60_neuron_32_1_39_s_89	11604137	(B) A bigger region of PlexB, PlexB  also binds to RhoA.	bind
7988	1	3542	6	11	NULL	NULL	NULL	CCT	GP		bind					tubulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_89_6_927_s_198	9200611	(B) A fraction of  CCT-bound  -tubulin acquires GTP binding competence in AMP - PNP.	bind
7989	2	3542	6	11	NULL	NULL	NULL	statement 1	Process		bind					GTP	Chemical				NULL	AMP-PNP	NULL	NULL	NULL	NULL	gw60_cell_89_6_927_s_198	9200611	(B) A fraction of  CCT-bound  -tubulin acquires GTP binding competence in AMP - PNP.	bind
11176	1	3542	7	11	NULL	NULL	NULL	CCT	GP		bind					tubulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_89_6_927_s_198	9200611	(B) A fraction of  CCT-bound  -tubulin acquires GTP binding competence in AMP - PNP.	bind
11177	2	3542	7	11	NULL	NULL	NULL	statement 1	Process		acquires					GTP	Chemical	competence for binding of			NULL	AMP - PNP	NULL	NULL	NULL	NULL	gw60_cell_89_6_927_s_198	9200611	(B) A fraction of  CCT-bound  -tubulin acquires GTP binding competence in AMP - PNP.	bind
80803	1	3542	11	NULL	NULL	0	NULL	CCT	NucleicAcidSubstance		binds to 					tubulin	Protein				NULL		0	NULL	NULL	NULL	gw60_cell_89_6_927_s_198	9200611	(B) A fraction of  CCT-bound  -tubulin acquires GTP binding competence in AMP - PNP.	bind
80804	2	3542	11	NULL	NULL	0	NULL	GTP	Chemical		binds to 					AMP - PNP	Chemical				NULL		0	NULL	NULL	NULL	gw60_cell_89_6_927_s_198	9200611	(B) A fraction of  CCT-bound  -tubulin acquires GTP binding competence in AMP - PNP.	bind
7990	1	3543	6	11	NULL	NULL	NULL	Fu monomer	GP		bind					Cos2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_23_10397_s_89	15542847	(B) A Fu monomer binds to Cos2 at the expense of Fu dimer formation.	bind
7991	2	3543	6	11	NULL	NULL	NULL	Fu	GP		forms a					dimer	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_23_10397_s_89	15542847	(B) A Fu monomer binds to Cos2 at the expense of Fu dimer formation.	bind
7992	3	3543	6	11	NULL	NULL	NULL	statement 1	Process		occurs at expense of					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_23_10397_s_89	15542847	(B) A Fu monomer binds to Cos2 at the expense of Fu dimer formation.	bind
11179	1	3543	7	11	NULL	NULL	NULL	Fu monomer	GP		binds					Cos2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_23_10397_s_89	15542847	(B) A Fu monomer binds to Cos2 at the expense of Fu dimer formation.	bind
11180	2	3543	7	11	NULL	NULL	NULL	Fu	GP		forms					dimer	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_23_10397_s_89	15542847	(B) A Fu monomer binds to Cos2 at the expense of Fu dimer formation.	bind
52977	3	3543	7	11	NULL	NULL	NULL	statement 1	Process		occurs at expense of					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_23_10397_s_89	15542847	(B) A Fu monomer binds to Cos2 at the expense of Fu dimer formation.	bind
80805	1	3543	11	NULL	NULL	0	NULL	Fu	Protein		forms					dimer	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_23_10397_s_89	15542847	(B) A Fu monomer binds to Cos2 at the expense of Fu dimer formation.	bind
80806	2	3543	11	NULL	NULL	0	NULL	Fu	Protein	monomer	binds to					Cos2	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_23_10397_s_89	15542847	(B) A Fu monomer binds to Cos2 at the expense of Fu dimer formation.	bind
80807	3	3543	11	NULL	NULL	0	NULL	statement 1	Process		leads to					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_23_10397_s_89	15542847	(B) A Fu monomer binds to Cos2 at the expense of Fu dimer formation.	bind
7993	1	3545	6	11	NULL	NULL	NULL	CREB peptide	GP	recombinant	bind					BDNF	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_neuron_20_4_727_s_144	9581764	(B) A recombinant CREB peptide can bind to the  BDNF promoter in a  CRE-dependent manner.	bind
7994	2	3545	6	11	NULL	NULL	NULL	statement 1	Process		is dependent on									CRE	NULL		NULL	NULL	NULL	NULL	gw60_neuron_20_4_727_s_144	9581764	(B) A recombinant CREB peptide can bind to the  BDNF promoter in a  CRE-dependent manner.	bind
11181	1	3545	7	11	NULL	NULL	NULL	CREB peptide	GP	recombinant	bind					BDNF	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_neuron_20_4_727_s_144	9581764	(B) A recombinant CREB peptide can bind to the  BDNF promoter in a  CRE-dependent manner.	bind
11182	2	3545	7	11	NULL	NULL	NULL	statement 1	Process		is dependent on									CRE	NULL		NULL	NULL	NULL	NULL	gw60_neuron_20_4_727_s_144	9581764	(B) A recombinant CREB peptide can bind to the  BDNF promoter in a  CRE-dependent manner.	bind
80808	1	3545	11	NULL	NULL	0	NULL	CREB peptide	PartOfProtein	recombinant 	binds to 					BDNF promoter	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_neuron_20_4_727_s_144	9581764	(B) A recombinant CREB peptide can bind to the  BDNF promoter in a  CRE-dependent manner.	bind
80809	2	3545	11	NULL	NULL	0	NULL	statement 1	Process		depends on					CRE	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_neuron_20_4_727_s_144	9581764	(B) A recombinant CREB peptide can bind to the  BDNF promoter in a  CRE-dependent manner.	bind
7995	1	3546	6	11	NULL	NULL	NULL	HEL	GP		bind					I-Ak	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_8_3_305_s_48	9529148	(B) A ribbon diagram ( Carson 1987  ) of HEL bound to I-Ak.	bind
11183	1	3546	7	11	NULL	NULL	NULL	HEL	GP		bind					I-Ak	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_8_3_305_s_48	9529148	(B) A ribbon diagram ( Carson 1987  ) of HEL bound to I-Ak.	bind
80810	1	3546	11	NULL	NULL	0	NULL	HEL	PartOfProtein		binds to 					I-Ak	Protein				NULL		0	NULL	NULL	NULL	gw60_immunity_8_3_305_s_48	9529148	(B) A ribbon diagram ( Carson 1987  ) of HEL bound to I-Ak.	bind
7996	1	3547	6	11	NULL	NULL	NULL				bind			Gi 1 subunit		GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_structure_4_11_1277_s_89	8939752	(b) A superposition of the C  traces of the Gi 1 subunit bound to GDP (blue), Gi 1bound to GTP  S-Mg2+ (red), and the GDP-Pi complex of G203AGi 1 (green).	bind
7997	2	3547	6	11	NULL	NULL	NULL				bind			Gi 1 subunit		GTP S-Mg+2	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_structure_4_11_1277_s_89	8939752	(b) A superposition of the C  traces of the Gi 1 subunit bound to GDP (blue), Gi 1bound to GTP  S-Mg2+ (red), and the GDP-Pi complex of G203AGi 1 (green).	bind
11184	1	3547	7	11	NULL	NULL	NULL				bind			Gi 1 subunit		GDP 	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_structure_4_11_1277_s_89	8939752	(b) A superposition of the C  traces of the Gi 1 subunit bound to GDP (blue), Gi 1bound to GTP  S-Mg2+ (red), and the GDP-Pi complex of G203AGi 1 (green).	bind
11185	2	3547	7	11	NULL	NULL	NULL				bind			Gi 1 subunit		GTP S-Mg2+ 	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_structure_4_11_1277_s_89	8939752	(b) A superposition of the C  traces of the Gi 1 subunit bound to GDP (blue), Gi 1bound to GTP  S-Mg2+ (red), and the GDP-Pi complex of G203AGi 1 (green).	bind
80811	1	3547	11	NULL	NULL	0	NULL	Gi 1 subunit	Protein		binds to 					GDP	Chemical				NULL		0	NULL	NULL	NULL	gw60_structure_4_11_1277_s_89	8939752	(b) A superposition of the C  traces of the Gi 1 subunit bound to GDP (blue), Gi 1bound to GTP  S-Mg2+ (red), and the GDP-Pi complex of G203AGi 1 (green).	bind
80812	2	3547	11	NULL	NULL	0	NULL	Gi	Protein		binds to 					GTP S-Mg2+	Chemical				NULL		0	NULL	NULL	NULL	gw60_structure_4_11_1277_s_89	8939752	(b) A superposition of the C  traces of the Gi 1 subunit bound to GDP (blue), Gi 1bound to GTP  S-Mg2+ (red), and the GDP-Pi complex of G203AGi 1 (green).	bind
80813	3	3547	11	NULL	NULL	0	NULL	GDP-Pi	Chemical		complex with 					G203AGi 1	Chemical				NULL		0	NULL	NULL	NULL	gw60_structure_4_11_1277_s_89	8939752	(b) A superposition of the C  traces of the Gi 1 subunit bound to GDP (blue), Gi 1bound to GTP  S-Mg2+ (red), and the GDP-Pi complex of G203AGi 1 (green).	bind
7999	1	3548	6	11	NULL	NULL	NULL	MCM3	GP		bind					chromatin	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_16_903_s_103	10469595	(b) A time-course experiment of the binding kinetics of MCM3 and Cdc6 to chromatin.	bind
8000	2	3548	6	11	NULL	NULL	NULL	Cdc6	GP		bind					chromatin	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_16_903_s_103	10469595	(b) A time-course experiment of the binding kinetics of MCM3 and Cdc6 to chromatin.	bind
11187	1	3548	7	11	NULL	NULL	NULL	MCM3	GP		bind					chromatin	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_16_903_s_103	10469595	(b) A time-course experiment of the binding kinetics of MCM3 and Cdc6 to chromatin.	bind
11188	2	3548	7	11	NULL	NULL	NULL	Cdc6	GP		bind					chromatin	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_16_903_s_103	10469595	(b) A time-course experiment of the binding kinetics of MCM3 and Cdc6 to chromatin.	bind
80814	1	3548	11	NULL	NULL	0	NULL	MCM3	Protein		binds to 					chromatin	Chromosome				NULL		0	NULL	NULL	NULL	gw60_currbiol_9_16_903_s_103	10469595	(b) A time-course experiment of the binding kinetics of MCM3 and Cdc6 to chromatin.	bind
80815	2	3548	11	NULL	NULL	NULL	NULL	Cdc6 	Protein		binds to 					chromatin	Chromosome				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_16_903_s_103	10469595	(b) A time-course experiment of the binding kinetics of MCM3 and Cdc6 to chromatin.	bind
8001	1	3549	6	11	NULL	NULL	NULL	lamin	GP	in vitro-translated;; Drosophila	bind					H2B peptides	GP	unmodified			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_17_1529_s_106	12225670	(B) A total of 3  l in vitro-translated  Drosophila lamin was bound to the unmodified (H2B) and acetylated (H2B-Ac) peptides.	bind
8002	2	3549	6	11	NULL	NULL	NULL	lamin	GP	in vitro-translated;; Drosophila	bind					H2B-Ac peptides	GP	acetylated			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_17_1529_s_106	12225670	(B) A total of 3  l in vitro-translated  Drosophila lamin was bound to the unmodified (H2B) and acetylated (H2B-Ac) peptides.	bind
52978	3	3549	6	11	NULL	NULL	NULL	H2B-Ac	GP		is					acetylated H2B peptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_17_1529_s_106	12225670	(B) A total of 3  l in vitro-translated  Drosophila lamin was bound to the unmodified (H2B) and acetylated (H2B-Ac) peptides.	bind
11189	1	3549	7	11	NULL	NULL	NULL	lamin	GP	in vitro-translated;; Drosophila	bind					H2B peptides	GP	unmodified			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_17_1529_s_106	12225670	(B) A total of 3  l in vitro-translated  Drosophila lamin was bound to the unmodified (H2B) and acetylated (H2B-Ac) peptides.	bind
11190	2	3549	7	11	NULL	NULL	NULL	lamin	GP	in vitro-translated;; Drosophila	bind					H2B-Ac peptides	GP	acetylated			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_17_1529_s_106	12225670	(B) A total of 3  l in vitro-translated  Drosophila lamin was bound to the unmodified (H2B) and acetylated (H2B-Ac) peptides.	bind
11191	3	3549	7	11	NULL	NULL	NULL	H2B-Ac	GP		is					acetylated H2B peptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_17_1529_s_106	12225670	(B) A total of 3  l in vitro-translated  Drosophila lamin was bound to the unmodified (H2B) and acetylated (H2B-Ac) peptides.	bind
80816	1	3549	11	NULL	NULL	0	NULL	 lamin	Protein	in vitro-translated;;Drosophila	binds to 					H2B peptide	PartOfProtein	unmodified			NULL		0	NULL	NULL	NULL	gw60_currbiol_12_17_1529_s_106	12225670	(B) A total of 3  l in vitro-translated  Drosophila lamin was bound to the unmodified (H2B) and acetylated (H2B-Ac) peptides.	bind
80817	2	3549	11	NULL	NULL	0	NULL	lamin	Protein	in vitro-translated;;Drosophila	binds to 					H2B-Ac peptide	PartOfProtein	acetylated			NULL		0	NULL	NULL	NULL	gw60_currbiol_12_17_1529_s_106	12225670	(B) A total of 3  l in vitro-translated  Drosophila lamin was bound to the unmodified (H2B) and acetylated (H2B-Ac) peptides.	bind
8003	1	3551	6	11	NULL	NULL	NULL	Abf1p	GP		bind					ADE5,7	NucleicAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_23_17_6279_s_81	12917348	(B) Abf1p binds in vitro to  ADE5, 7 but not to  IMD2.	bind
8005	2	3551	6	11	NULL	NULL	NULL	Abf1p	GP		does not bind					IMD2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_17_6279_s_81	12917348	(B) Abf1p binds in vitro to  ADE5, 7 but not to  IMD2.	bind
11192	1	3551	7	11	NULL	NULL	NULL	Abf1p	GP		binds					ADE5,7	NucleicAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_23_17_6279_s_81	12917348	(B) Abf1p binds in vitro to  ADE5, 7 but not to  IMD2.	bind
11193	2	3551	7	11	NULL	NULL	NULL	Abf1p	GP		does not bind					IMD2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_17_6279_s_81	12917348	(B) Abf1p binds in vitro to  ADE5, 7 but not to  IMD2.	bind
80818	1	3551	11	NULL	NULL	0	NULL	Abf1p	Protein		binds to 					ADE5,7	NucleicAcidSubstance				NULL	in vitro	0	NULL	NULL	NULL	gw60_molcellbiol_23_17_6279_s_81	12917348	(B) Abf1p binds in vitro to  ADE5, 7 but not to  IMD2.	bind
80819	2	3551	11	NULL	NULL	0	NULL	Abf1p	Protein		does not bind to						Gene				NULL	in vitro	0	NULL	NULL	NULL	gw60_molcellbiol_23_17_6279_s_81	12917348	(B) Abf1p binds in vitro to  ADE5, 7 but not to  IMD2.	bind
8006	1	3552	6	11	NULL	NULL	NULL	Rac1	GP		bind					GST-PAK	GP		GBD		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_79	10508610	(b) Ability of Rac1 and Cdc42 17-32 peptides to compete for the binding of Rac1 and Cdc42 to GST-PAK GTPase-binding domains (GBD).	bind
8007	2	3552	6	11	NULL	NULL	NULL	Cdc42	GP		bind					GST-PAK	GP		GBD		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_79	10508610	(b) Ability of Rac1 and Cdc42 17-32 peptides to compete for the binding of Rac1 and Cdc42 to GST-PAK GTPase-binding domains (GBD).	bind
8008	3	3552	6	11	NULL	NULL	NULL	GBD	GP		is					GTPase-binding domain	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_79	10508610	(b) Ability of Rac1 and Cdc42 17-32 peptides to compete for the binding of Rac1 and Cdc42 to GST-PAK GTPase-binding domains (GBD).	bind
8009	4	3552	6	11	NULL	NULL	NULL	Rac1 peptides	GP		bind					GST-PAK	GP		GBD		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_79	10508610	(b) Ability of Rac1 and Cdc42 17-32 peptides to compete for the binding of Rac1 and Cdc42 to GST-PAK GTPase-binding domains (GBD).	bind
8010	5	3552	6	11	NULL	NULL	NULL	statement 4	Process		competes with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_79	10508610	(b) Ability of Rac1 and Cdc42 17-32 peptides to compete for the binding of Rac1 and Cdc42 to GST-PAK GTPase-binding domains (GBD).	bind
8011	6	3552	6	11	NULL	NULL	NULL	Cdc42 	GP		bind			17-32 peptide		GST-PAK	GP		GBD		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_79	10508610	(b) Ability of Rac1 and Cdc42 17-32 peptides to compete for the binding of Rac1 and Cdc42 to GST-PAK GTPase-binding domains (GBD).	bind
8012	7	3552	6	11	NULL	NULL	NULL	statement 6	Process		competes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_79	10508610	(b) Ability of Rac1 and Cdc42 17-32 peptides to compete for the binding of Rac1 and Cdc42 to GST-PAK GTPase-binding domains (GBD).	bind
11194	1	3552	7	11	NULL	NULL	NULL	Rac1	GP		bind					GST-PAK	GP		GBD		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_79	10508610	(b) Ability of Rac1 and Cdc42 17-32 peptides to compete for the binding of Rac1 and Cdc42 to GST-PAK GTPase-binding domains (GBD).	bind
11195	2	3552	7	11	NULL	NULL	NULL	Cdc42	GP		bind					GST-PAK	GP		GBD		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_79	10508610	(b) Ability of Rac1 and Cdc42 17-32 peptides to compete for the binding of Rac1 and Cdc42 to GST-PAK GTPase-binding domains (GBD).	bind
11196	3	3552	7	11	NULL	NULL	NULL	Rac1 peptide	GP		bind					GST-PAK	GP		GBD		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_79	10508610	(b) Ability of Rac1 and Cdc42 17-32 peptides to compete for the binding of Rac1 and Cdc42 to GST-PAK GTPase-binding domains (GBD).	bind
11197	4	3552	7	11	NULL	NULL	NULL	GTPase-binding domain	GP		is					GBD	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_79	10508610	(b) Ability of Rac1 and Cdc42 17-32 peptides to compete for the binding of Rac1 and Cdc42 to GST-PAK GTPase-binding domains (GBD).	bind
52980	5	3552	7	11	NULL	NULL	NULL	statement 3	Process		competes with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_79	10508610	(b) Ability of Rac1 and Cdc42 17-32 peptides to compete for the binding of Rac1 and Cdc42 to GST-PAK GTPase-binding domains (GBD).	bind
52981	6	3552	7	11	NULL	NULL	NULL	Cdc42 peptides	GP		bind			17-32		GST-PAK	GP		GBD		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_79	10508610	(b) Ability of Rac1 and Cdc42 17-32 peptides to compete for the binding of Rac1 and Cdc42 to GST-PAK GTPase-binding domains (GBD).	bind
52982	7	3552	7	11	NULL	NULL	NULL	statement 6	Process		competes with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_79	10508610	(b) Ability of Rac1 and Cdc42 17-32 peptides to compete for the binding of Rac1 and Cdc42 to GST-PAK GTPase-binding domains (GBD).	bind
80820	1	3552	11	NULL	NULL	0	NULL	GST-PAK 	Protein		binds to 			GTPase-binding domain		Rac1	Protein				NULL		0	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_79	10508610	(b) Ability of Rac1 and Cdc42 17-32 peptides to compete for the binding of Rac1 and Cdc42 to GST-PAK GTPase-binding domains (GBD).	bind
80821	2	3552	11	NULL	NULL	0	NULL	GST-PAK	Protein		binds to 			GTPase-binding domain		Cdc42	Protein				NULL		0	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_79	10508610	(b) Ability of Rac1 and Cdc42 17-32 peptides to compete for the binding of Rac1 and Cdc42 to GST-PAK GTPase-binding domains (GBD).	bind
80822	3	3552	11	NULL	NULL	0	NULL	GTPase-binding domain	PartOfProtein		is					GBD	PartOfProtein				NULL		0	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_79	10508610	(b) Ability of Rac1 and Cdc42 17-32 peptides to compete for the binding of Rac1 and Cdc42 to GST-PAK GTPase-binding domains (GBD).	bind
8014	1	3554	6	11	NULL	NULL	NULL	HS1	GP		bind			actin binding domain		PIP2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_3829_s_202	9632767	(B) Actin-binding domain of HS1 binds PIP2.	bind
11198	1	3554	7	11	NULL	NULL	NULL	HS1	GP		binds			Actin-binding domain		 PIP2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_3829_s_202	9632767	(B) Actin-binding domain of HS1 binds PIP2.	bind
80828	1	3554	11	NULL	NULL	NULL	NULL	HS1	Protein		binds to 			Actin-binding domain		PIP2	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_3829_s_202	9632767	(B) Actin-binding domain of HS1 binds PIP2.	bind
8077	1	3556	6	11	NULL	NULL	NULL	PI3K-C2	GP	deletion of	stimulates			N-terminal clathrin binding region		PI3K-C2	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_2_443_s_70	11239472	(b) Activity of PI3K-C2  is greatly stimulated by deletion of the N-terminal clathrin binding region of PI3K-C2  (stippled bar).	bind
11199	1	3556	7	11	NULL	NULL	NULL	PI3K-C2	GP	activity of	is stimulated by					PI3K-C2	GP	deletion of	N-terminal clathrin binding region		NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_2_443_s_70	11239472	(b) Activity of PI3K-C2  is greatly stimulated by deletion of the N-terminal clathrin binding region of PI3K-C2  (stippled bar).	bind
80834	1	3556	11	NULL	NULL	0	NULL	PI3K-C2	Protein		has binding site for			N-terminal 		clathrin	Protein				NULL		0	NULL	NULL	NULL	gw60_molcell_7_2_443_s_70	11239472	(b) Activity of PI3K-C2  is greatly stimulated by deletion of the N-terminal clathrin binding region of PI3K-C2  (stippled bar).	bind
80835	2	3556	11	NULL	NULL	0	NULL	PI3K-C2	Protein		undergoes			N-terminal clathrin binding region		deletion	MolecularProcess				NULL		0	NULL	NULL	NULL	gw60_molcell_7_2_443_s_70	11239472	(b) Activity of PI3K-C2  is greatly stimulated by deletion of the N-terminal clathrin binding region of PI3K-C2  (stippled bar).	bind
80836	3	3556	11	NULL	NULL	0	NULL	statement 2	Process		activates					PI3K-C2	Protein				NULL		0	NULL	NULL	NULL	gw60_molcell_7_2_443_s_70	11239472	(b) Activity of PI3K-C2  is greatly stimulated by deletion of the N-terminal clathrin binding region of PI3K-C2  (stippled bar).	bind
8078	1	3557	6	11	NULL	NULL	NULL	Ad2	GP		bind			E1B		PCAF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5540_s_300	10891493	(B) Ad2 E1B binds to PCAF.	bind
11200	1	3557	7	11	NULL	NULL	NULL	Ad2 	GP		binds			E1B		PCAF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5540_s_300	10891493	(B) Ad2 E1B binds to PCAF.	bind
80837	1	3557	11	NULL	NULL	0	NULL	Ad2 E1B	Protein		binds to 					PCAF	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_15_5540_s_300	10891493	(B) Ad2 E1B binds to PCAF.	bind
8079	1	3558	6	11	NULL	NULL	NULL	uPA	GP		bind					uPAR	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_367_s_141	16267271	(B) Addition of R3 (monoclonal anti-uPAR antibody blocking uPA binding to  uPAR) blocks uPA-induced migration of both wt- and  hcr-uPAR-expressing cells.	bind
8080	2	3558	6	11	NULL	NULL	NULL	R3	GP		is 					anti-uPAR	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_367_s_141	16267271	(B) Addition of R3 (monoclonal anti-uPAR antibody blocking uPA binding to  uPAR) blocks uPA-induced migration of both wt- and  hcr-uPAR-expressing cells.	bind
8081	3	3558	6	11	NULL	NULL	NULL	R3	GP		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_367_s_141	16267271	(B) Addition of R3 (monoclonal anti-uPAR antibody blocking uPA binding to  uPAR) blocks uPA-induced migration of both wt- and  hcr-uPAR-expressing cells.	bind
8082	4	3558	6	11	NULL	NULL	NULL	uPA	GP		induces					uPAR-expressing cells	Cell	wt;; migration of			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_367_s_141	16267271	(B) Addition of R3 (monoclonal anti-uPAR antibody blocking uPA binding to  uPAR) blocks uPA-induced migration of both wt- and  hcr-uPAR-expressing cells.	bind
8083	5	3558	6	11	NULL	NULL	NULL	uPA	GP		induces					hcr-uPAR-expressing cells	Cell	migration of			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_367_s_141	16267271	(B) Addition of R3 (monoclonal anti-uPAR antibody blocking uPA binding to  uPAR) blocks uPA-induced migration of both wt- and  hcr-uPAR-expressing cells.	bind
8084	6	3558	6	11	NULL	NULL	NULL	R3	GP	addition of	blocks					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_367_s_141	16267271	(B) Addition of R3 (monoclonal anti-uPAR antibody blocking uPA binding to  uPAR) blocks uPA-induced migration of both wt- and  hcr-uPAR-expressing cells.	bind
8085	7	3558	6	11	NULL	NULL	NULL	R3	GP	addition of	blocks					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_367_s_141	16267271	(B) Addition of R3 (monoclonal anti-uPAR antibody blocking uPA binding to  uPAR) blocks uPA-induced migration of both wt- and  hcr-uPAR-expressing cells.	bind
40778	8	3558	6	11	NULL	NULL	NULL	anti-uPAR	GP		is a type of					monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_367_s_141	16267271	(B) Addition of R3 (monoclonal anti-uPAR antibody blocking uPA binding to  uPAR) blocks uPA-induced migration of both wt- and  hcr-uPAR-expressing cells.	bind
11201	1	3558	7	11	NULL	NULL	NULL	uPA	GP		bind					uPAR	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_367_s_141	16267271	(B) Addition of R3 (monoclonal anti-uPAR antibody blocking uPA binding to  uPAR) blocks uPA-induced migration of both wt- and  hcr-uPAR-expressing cells.	bind
11202	2	3558	7	11	NULL	NULL	NULL	monoclonal anti-uPAR antibody	GP		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_367_s_141	16267271	(B) Addition of R3 (monoclonal anti-uPAR antibody blocking uPA binding to  uPAR) blocks uPA-induced migration of both wt- and  hcr-uPAR-expressing cells.	bind
11203	3	3558	7	11	NULL	NULL	NULL	uPA	GP		induce					uPAR-expressing cells	Cell	migration of;;wt			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_367_s_141	16267271	(B) Addition of R3 (monoclonal anti-uPAR antibody blocking uPA binding to  uPAR) blocks uPA-induced migration of both wt- and  hcr-uPAR-expressing cells.	bind
11204	4	3558	7	11	NULL	NULL	NULL	uPA	GP		induce					hcr-uPAR-expressing cells	Cell	migration of			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_367_s_141	16267271	(B) Addition of R3 (monoclonal anti-uPAR antibody blocking uPA binding to  uPAR) blocks uPA-induced migration of both wt- and  hcr-uPAR-expressing cells.	bind
11205	5	3558	7	11	NULL	NULL	NULL	R3	GP	addition of	blocks					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_367_s_141	16267271	(B) Addition of R3 (monoclonal anti-uPAR antibody blocking uPA binding to  uPAR) blocks uPA-induced migration of both wt- and  hcr-uPAR-expressing cells.	bind
11206	6	3558	7	11	NULL	NULL	NULL	R3	GP	addition of	blocks					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_367_s_141	16267271	(B) Addition of R3 (monoclonal anti-uPAR antibody blocking uPA binding to  uPAR) blocks uPA-induced migration of both wt- and  hcr-uPAR-expressing cells.	bind
52983	7	3558	7	11	NULL	NULL	NULL	R3	GP		is					anti-uPAR	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_367_s_141	16267271	(B) Addition of R3 (monoclonal anti-uPAR antibody blocking uPA binding to  uPAR) blocks uPA-induced migration of both wt- and  hcr-uPAR-expressing cells.	bind
52984	8	3558	7	11	NULL	NULL	NULL	anti-uPAR	GP		is a type of					monoclonal antibody \t	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_367_s_141	16267271	(B) Addition of R3 (monoclonal anti-uPAR antibody blocking uPA binding to  uPAR) blocks uPA-induced migration of both wt- and  hcr-uPAR-expressing cells.	bind
80840	1	3558	11	NULL	NULL	0	NULL	uPA	Protein		binds to 					uPAR	Protein				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_1_367_s_141	16267271	(B) Addition of R3 (monoclonal anti-uPAR antibody blocking uPA binding to  uPAR) blocks uPA-induced migration of both wt- and  hcr-uPAR-expressing cells.	bind
80841	2	3558	11	NULL	NULL	0	NULL	anti-uPAR antibody	PartOfProtein	monoclonal	blocks					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_1_367_s_141	16267271	(B) Addition of R3 (monoclonal anti-uPAR antibody blocking uPA binding to  uPAR) blocks uPA-induced migration of both wt- and  hcr-uPAR-expressing cells.	bind
80842	3	3558	11	NULL	NULL	0	NULL	R3	PartOfProtein		is					anti-uPAR antibody	PartOfProtein	monoclonal			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_1_367_s_141	16267271	(B) Addition of R3 (monoclonal anti-uPAR antibody blocking uPA binding to  uPAR) blocks uPA-induced migration of both wt- and  hcr-uPAR-expressing cells.	bind
80843	4	3558	11	NULL	NULL	NULL	NULL	cells	cell	hcr-uPAR-expressing	undergoes					migration	BiologicalProcess				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_367_s_141	16267271	(B) Addition of R3 (monoclonal anti-uPAR antibody blocking uPA binding to  uPAR) blocks uPA-induced migration of both wt- and  hcr-uPAR-expressing cells.	bind
80845	5	3558	11	NULL	NULL	0	NULL	cells	cell	wt-uPAR-expressing	undergoes					migration	BiologicalProcess				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_1_367_s_141	16267271	(B) Addition of R3 (monoclonal anti-uPAR antibody blocking uPA binding to  uPAR) blocks uPA-induced migration of both wt- and  hcr-uPAR-expressing cells.	bind
80846	6	3558	11	NULL	NULL	0	NULL	uPA	Protein		induces					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_1_367_s_141	16267271	(B) Addition of R3 (monoclonal anti-uPAR antibody blocking uPA binding to  uPAR) blocks uPA-induced migration of both wt- and  hcr-uPAR-expressing cells.	bind
80847	7	3558	11	NULL	NULL	0	NULL	uPA	Protein		induces					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_1_367_s_141	16267271	(B) Addition of R3 (monoclonal anti-uPAR antibody blocking uPA binding to  uPAR) blocks uPA-induced migration of both wt- and  hcr-uPAR-expressing cells.	bind
80848	8	3558	11	NULL	NULL	0	NULL	R3	PartOfProtein		blocks					statement 6	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_1_367_s_141	16267271	(B) Addition of R3 (monoclonal anti-uPAR antibody blocking uPA binding to  uPAR) blocks uPA-induced migration of both wt- and  hcr-uPAR-expressing cells.	bind
80849	9	3558	11	NULL	NULL	0	NULL	R3	PartOfProtein		blocks					statement 7	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_1_367_s_141	16267271	(B) Addition of R3 (monoclonal anti-uPAR antibody blocking uPA binding to  uPAR) blocks uPA-induced migration of both wt- and  hcr-uPAR-expressing cells.	bind
8086	1	3559	6	11	NULL	NULL	NULL	R1/1	GP		bind					ICAM-1	GP		D1		NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_74_2_830_s_135	16428725	(B) Adhesion of NTHI was also determined  after incubating CHO-ICAM-1 cells with MAbs R1/1 and 8.4A6, which bind ICAM-1 D1  and D2, respectively.	bind
8087	2	3559	6	11	NULL	NULL	NULL	8.4A6	GP		bind					ICAM-1	GP		D2		NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_74_2_830_s_135	16428725	(B) Adhesion of NTHI was also determined  after incubating CHO-ICAM-1 cells with MAbs R1/1 and 8.4A6, which bind ICAM-1 D1  and D2, respectively.	bind
52985	3	3559	6	10	NULL	0	NULL	R1/1	NULL		is a type of	NULL				monoclonal antibody	NULL				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_74_2_830_s_135	16428725	(B) Adhesion of NTHI was also determined  after incubating CHO-ICAM-1 cells with MAbs R1/1 and 8.4A6, which bind ICAM-1 D1  and D2, respectively.	bind
52986	4	3559	6	10	NULL	0	NULL	8.4A6	NULL		is a type of	NULL				monoclonal antibody	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_74_2_830_s_135	16428725	(B) Adhesion of NTHI was also determined  after incubating CHO-ICAM-1 cells with MAbs R1/1 and 8.4A6, which bind ICAM-1 D1  and D2, respectively.	bind
11207	1	3559	7	NULL	NULL	0	NULL	R1/1 	NULL		bind	NULL				ICAM-1 	NULL		D1		NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_74_2_830_s_135	16428725	(B) Adhesion of NTHI was also determined  after incubating CHO-ICAM-1 cells with MAbs R1/1 and 8.4A6, which bind ICAM-1 D1  and D2, respectively.	bind
11208	2	3559	7	NULL	NULL	0	NULL	8.4A6	NULL		bind	NULL				ICAM-1	NULL		D2		NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_74_2_830_s_135	16428725	(B) Adhesion of NTHI was also determined  after incubating CHO-ICAM-1 cells with MAbs R1/1 and 8.4A6, which bind ICAM-1 D1  and D2, respectively.	bind
52987	3	3559	7	10	NULL	0	NULL	R1/1	NULL		is a type of	NULL				monoclonal antibody	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_74_2_830_s_135	16428725	(B) Adhesion of NTHI was also determined  after incubating CHO-ICAM-1 cells with MAbs R1/1 and 8.4A6, which bind ICAM-1 D1  and D2, respectively.	bind
52988	4	3559	7	10	NULL	0	NULL	8.4A6	NULL		is a type of	NULL				monoclonal antibody	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_74_2_830_s_135	16428725	(B) Adhesion of NTHI was also determined  after incubating CHO-ICAM-1 cells with MAbs R1/1 and 8.4A6, which bind ICAM-1 D1  and D2, respectively.	bind
80873	1	3559	11	NULL	NULL	0	NULL	MAbs R1/1	PartOfProtein		binds to 					ICAM-1 D1	Protein				NULL		0	NULL	NULL	NULL	gw70_infectimmun_74_2_830_s_135	16428725	(B) Adhesion of NTHI was also determined  after incubating CHO-ICAM-1 cells with MAbs R1/1 and 8.4A6, which bind ICAM-1 D1  and D2, respectively.	bind
80874	2	3559	11	NULL	NULL	0	NULL	8.4A6	PartOfProtein		binds to 					ICAM-1 D2	Protein				NULL		0	NULL	NULL	NULL	gw70_infectimmun_74_2_830_s_135	16428725	(B) Adhesion of NTHI was also determined  after incubating CHO-ICAM-1 cells with MAbs R1/1 and 8.4A6, which bind ICAM-1 D1  and D2, respectively.	bind
8088	1	3563	6	11	NULL	NULL	NULL	Myc-Pak1	GP		bind					Nck	GP				NULL	COS-7 cell lysates	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_22_8058_s_283	14585966	(B) Akt expression in  COS-7 cells leads to reduced binding of Myc-Pak1 with Nck in a GST-Nck pull-down  assay with cell lysates.	bind
8089	2	3563	6	11	NULL	NULL	NULL	Akt	GP	expression of	reduces					statement 1	Process				NULL	COS-7 cell lysates	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_22_8058_s_283	14585966	(B) Akt expression in  COS-7 cells leads to reduced binding of Myc-Pak1 with Nck in a GST-Nck pull-down  assay with cell lysates.	bind
11213	1	3563	7	11	NULL	NULL	NULL	Myc-Pak1	GP		bind					Nck	GP				NULL	COS-7 cells lysates	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_22_8058_s_283	14585966	(B) Akt expression in  COS-7 cells leads to reduced binding of Myc-Pak1 with Nck in a GST-Nck pull-down  assay with cell lysates.	bind
11214	2	3563	7	11	NULL	NULL	NULL	Akt	GP	expression of	reduces					statement 1	Process				NULL	COS-7 cells lysates	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_22_8058_s_283	14585966	(B) Akt expression in  COS-7 cells leads to reduced binding of Myc-Pak1 with Nck in a GST-Nck pull-down  assay with cell lysates.	bind
80875	1	3563	11	NULL	NULL	0	NULL	Myc-Pak1	Protein		binds to 					Nck	Protein				NULL	GST-Nck pull-down assay	0	NULL	NULL	NULL	gw70_molcellbiol_23_22_8058_s_283	14585966	(B) Akt expression in  COS-7 cells leads to reduced binding of Myc-Pak1 with Nck in a GST-Nck pull-down  assay with cell lysates.	bind
80876	2	3563	11	NULL	NULL	0	NULL	Akt	Protein		expressed on					COS-7 cells	Cell				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_22_8058_s_283	14585966	(B) Akt expression in  COS-7 cells leads to reduced binding of Myc-Pak1 with Nck in a GST-Nck pull-down  assay with cell lysates.	bind
80877	3	3563	11	NULL	NULL	0	NULL	statement 2	Process		reduces					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_22_8058_s_283	14585966	(B) Akt expression in  COS-7 cells leads to reduced binding of Myc-Pak1 with Nck in a GST-Nck pull-down  assay with cell lysates.	bind
8090	1	3564	6	11	NULL	NULL	NULL	Rac	GP		bind					PAK	GP		PBD		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_4_749_s_59	14765121	(B) AlF treatment causes increased binding of Rac to the p21-binding domain  of PAK (PAK PBD).	bind
8091	2	3564	6	11	NULL	NULL	NULL	AIF	GP		increases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_4_749_s_59	14765121	(B) AlF treatment causes increased binding of Rac to the p21-binding domain  of PAK (PAK PBD).	bind
8092	3	3564	6	11	NULL	NULL	NULL	PBD	GP		is					p21-binding domain	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_4_749_s_59	14765121	(B) AlF treatment causes increased binding of Rac to the p21-binding domain  of PAK (PAK PBD).	bind
11218	1	3564	7	11	NULL	NULL	NULL	Rac	GP		bind					PAK	GP		PBD		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_4_749_s_59	14765121	(B) AlF treatment causes increased binding of Rac to the p21-binding domain  of PAK (PAK PBD).	bind
11219	2	3564	7	11	NULL	NULL	NULL	AlF	GP		increase					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_4_749_s_59	14765121	(B) AlF treatment causes increased binding of Rac to the p21-binding domain  of PAK (PAK PBD).	bind
11221	3	3564	7	11	NULL	NULL	NULL	PBD	GP		is					p21-binding domain	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_4_749_s_59	14765121	(B) AlF treatment causes increased binding of Rac to the p21-binding domain  of PAK (PAK PBD).	bind
80878	1	3564	11	NULL	NULL	0	NULL	Rac	Protein		binds to 					PAK	Protein		p21-binding domain		NULL		0	NULL	NULL	NULL	gw70_embo_23_4_749_s_59	14765121	(B) AlF treatment causes increased binding of Rac to the p21-binding domain  of PAK (PAK PBD).	bind
80879	2	3564	11	NULL	NULL	0	NULL	AlF	Chemical		increases					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_embo_23_4_749_s_59	14765121	(B) AlF treatment causes increased binding of Rac to the p21-binding domain  of PAK (PAK PBD).	bind
80880	3	3564	11	NULL	NULL	0	NULL	PAK	Protein		is			p21-binding domain		PAK PBD	Protein				NULL		0	NULL	NULL	NULL	gw70_embo_23_4_749_s_59	14765121	(B) AlF treatment causes increased binding of Rac to the p21-binding domain  of PAK (PAK PBD).	bind
8093	1	3565	6	11	NULL	NULL	NULL	target genes	GP	mouse	bind				sox-oct cis elements	Sox2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_14_6031_s_192	15988017	(B) Alignment of  the composite sox-oct  cis elements from the respective mouse target genes that are known to bind Sox2 and Oct4,  including that described in this paper and present in the CR4-B region in panel A  (complementary strand).	bind
8094	2	3565	6	11	NULL	NULL	NULL	target genes	GP	mouse	bind				sox-oct cis elements	Oct4	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_14_6031_s_192	15988017	(B) Alignment of  the composite sox-oct  cis elements from the respective mouse target genes that are known to bind Sox2 and Oct4,  including that described in this paper and present in the CR4-B region in panel A  (complementary strand).	bind
11226	1	3565	7	11	NULL	NULL	NULL	target genes	GP	mouse	bind				sox-oct cis elements	Sox2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_14_6031_s_192	15988017	(B) Alignment of  the composite sox-oct  cis elements from the respective mouse target genes that are known to bind Sox2 and Oct4,  including that described in this paper and present in the CR4-B region in panel A  (complementary strand).	bind
11229	2	3565	7	11	NULL	NULL	NULL	target genes	GP	mouse	bind				sox-oct cis elements	Oct4	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_14_6031_s_192	15988017	(B) Alignment of  the composite sox-oct  cis elements from the respective mouse target genes that are known to bind Sox2 and Oct4,  including that described in this paper and present in the CR4-B region in panel A  (complementary strand).	bind
8095	1	3571	6	11	NULL	NULL	NULL	EKLF	GP	mutant	bind			amino-terminal 		betamaj	NucleicAcid	cognate		CACC motif	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_1_161_s_187	11739731	(B) All amino-terminal mutants of EKLF bind the cognate betamaj CACC motif.	bind
11236	1	3571	7	11	NULL	NULL	NULL	EKLF	GP	 mutant	bind			amino-terminal		betamaj	NucleicAcid	cognate		CACC motif	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_1_161_s_187	11739731	(B) All amino-terminal mutants of EKLF bind the cognate betamaj CACC motif.	bind
80881	1	3571	11	NULL	NULL	0	NULL	EKLF	Protein	mutants	binds to 			amino-terminal		betamaj	Protein		CACC motif		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_1_161_s_187	11739731	(B) All amino-terminal mutants of EKLF bind the cognate betamaj CACC motif.	bind
8175	1	3573	6	11	NULL	NULL	NULL	Ran	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_65_4_570_s_209	11729264	(B) Amino acid sequence of Ran showing the  Switch 1 and  Switch 2 regions that undergo a conformational switch between the GTP and GDP binding states, and  the basic patch.	bind
8176	2	3573	6	11	NULL	NULL	NULL	Ran	GP		bind					GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_65_4_570_s_209	11729264	(B) Amino acid sequence of Ran showing the  Switch 1 and  Switch 2 regions that undergo a conformational switch between the GTP and GDP binding states, and  the basic patch.	bind
8177	3	3573	6	11	NULL	NULL	NULL	statement 1	Process		changes					Ran	GP	conformation of 			NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_65_4_570_s_209	11729264	(B) Amino acid sequence of Ran showing the  Switch 1 and  Switch 2 regions that undergo a conformational switch between the GTP and GDP binding states, and  the basic patch.	bind
8178	4	3573	6	11	NULL	NULL	NULL	statement 2	Process		changes					Ran	GP	conformation of 			NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_65_4_570_s_209	11729264	(B) Amino acid sequence of Ran showing the  Switch 1 and  Switch 2 regions that undergo a conformational switch between the GTP and GDP binding states, and  the basic patch.	bind
8301	5	3573	6	11	NULL	NULL	NULL	Ran	GP		undergoes			Switch 1		conformational change	Process				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_65_4_570_s_209	11729264	(B) Amino acid sequence of Ran showing the  Switch 1 and  Switch 2 regions that undergo a conformational switch between the GTP and GDP binding states, and  the basic patch.	bind
8302	6	3573	6	11	NULL	NULL	NULL	Ran	GP		undergoes			Switch 2		conformational change	Process				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_65_4_570_s_209	11729264	(B) Amino acid sequence of Ran showing the  Switch 1 and  Switch 2 regions that undergo a conformational switch between the GTP and GDP binding states, and  the basic patch.	bind
11331	1	3573	7	11	NULL	NULL	NULL	Ran	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_65_4_570_s_209	11729264	(B) Amino acid sequence of Ran showing the  Switch 1 and  Switch 2 regions that undergo a conformational switch between the GTP and GDP binding states, and  the basic patch.	bind
11332	2	3573	7	11	NULL	NULL	NULL	Ran	GP		bind					GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_65_4_570_s_209	11729264	(B) Amino acid sequence of Ran showing the  Switch 1 and  Switch 2 regions that undergo a conformational switch between the GTP and GDP binding states, and  the basic patch.	bind
11333	3	3573	7	11	NULL	NULL	NULL	Ran	GP		undergoes			switch 1 region		conformational change	Process				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_65_4_570_s_209	11729264	(B) Amino acid sequence of Ran showing the  Switch 1 and  Switch 2 regions that undergo a conformational switch between the GTP and GDP binding states, and  the basic patch.	bind
11334	4	3573	7	11	NULL	NULL	NULL	Ran	GP		undergoes			switch 2 region		conformational change	Process				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_65_4_570_s_209	11729264	(B) Amino acid sequence of Ran showing the  Switch 1 and  Switch 2 regions that undergo a conformational switch between the GTP and GDP binding states, and  the basic patch.	bind
11335	5	3573	7	11	NULL	NULL	NULL	statement 1	Process		changes					Ran	GP	conformation of			NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_65_4_570_s_209	11729264	(B) Amino acid sequence of Ran showing the  Switch 1 and  Switch 2 regions that undergo a conformational switch between the GTP and GDP binding states, and  the basic patch.	bind
11336	6	3573	7	11	NULL	NULL	NULL	statement 2	Process		changes					Ran	GP	conformation of			NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_65_4_570_s_209	11729264	(B) Amino acid sequence of Ran showing the  Switch 1 and  Switch 2 regions that undergo a conformational switch between the GTP and GDP binding states, and  the basic patch.	bind
8098	1	3574	6	11	NULL	NULL	NULL	Tem1	GP		bind					Cdc15	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_5_697_s_200	12628189	(B) Amn1 regulates the binding between Tem1 and Cdc15.	bind
8099	2	3574	6	11	NULL	NULL	NULL	Amn1	GP		regulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_5_697_s_200	12628189	(B) Amn1 regulates the binding between Tem1 and Cdc15.	bind
11239	1	3574	7	11	NULL	NULL	NULL	Tem1	GP		bind					Cdc15	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_5_697_s_200	12628189	(B) Amn1 regulates the binding between Tem1 and Cdc15.	bind
11240	2	3574	7	11	NULL	NULL	NULL	Amn1	GP		regulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_5_697_s_200	12628189	(B) Amn1 regulates the binding between Tem1 and Cdc15.	bind
80882	1	3574	11	NULL	NULL	0	NULL	Tem1	Protein		binds to 					Cdc15	Protein				NULL		0	NULL	NULL	NULL	gw60_cell_112_5_697_s_200	12628189	(B) Amn1 regulates the binding between Tem1 and Cdc15.	bind
80883	2	3574	11	NULL	NULL	0	NULL	Amn1	Protein		regulates					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_cell_112_5_697_s_200	12628189	(B) Amn1 regulates the binding between Tem1 and Cdc15.	bind
8101	1	3575	6	11	NULL	NULL	NULL	L-ficolin	Chemical		bind					T-1	Organism				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_2_1052_s_161	15664949	(B) Amounts of L-ficolin bound to T-1 and Wood.	bind
8102	2	3575	6	11	NULL	NULL	NULL	L-ficolin	Chemical		bind					Wood	Organism				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_2_1052_s_161	15664949	(B) Amounts of L-ficolin bound to T-1 and Wood.	bind
11243	1	3575	7	11	NULL	NULL	NULL	L-ficolin	Chemical		bind					T-1	Organism				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_2_1052_s_161	15664949	(B) Amounts of L-ficolin bound to T-1 and Wood.	bind
11246	2	3575	7	11	NULL	NULL	NULL	L-ficolin	Chemical		bind					Wood	Organism				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_2_1052_s_161	15664949	(B) Amounts of L-ficolin bound to T-1 and Wood.	bind
80884	1	3575	11	NULL	NULL	0	NULL	L-ficolin	Protein		binds to 					T-1	Organism				NULL		0	NULL	NULL	NULL	gw70_infectimmun_73_2_1052_s_161	15664949	(B) Amounts of L-ficolin bound to T-1 and Wood.	bind
80885	2	3575	11	NULL	NULL	0	NULL	L-ficolin	Protein		binds to 					Wood	Organism				NULL		0	NULL	NULL	NULL	gw70_infectimmun_73_2_1052_s_161	15664949	(B) Amounts of L-ficolin bound to T-1 and Wood.	bind
8103	1	3577	6	11	NULL	NULL	NULL	neutrophil collagenase 	GP	active	bind					collagen	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_5_2319_s_233	10225890	(B) Analysis of active and latent forms of neutrophil collagenase binding to collagen.	bind
8104	2	3577	6	11	NULL	NULL	NULL	neutrophil collagenase 	GP	latent	bind					collagen	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_5_2319_s_233	10225890	(B) Analysis of active and latent forms of neutrophil collagenase binding to collagen.	bind
11252	1	3577	7	11	NULL	NULL	NULL	neutrophil collagenase	GP	active	bind					collagen	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_5_2319_s_233	10225890	(B) Analysis of active and latent forms of neutrophil collagenase binding to collagen.	bind
11254	2	3577	7	11	NULL	NULL	NULL	neutrophil collagenase	GP	latent	bind					collagen	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_5_2319_s_233	10225890	(B) Analysis of active and latent forms of neutrophil collagenase binding to collagen.	bind
80886	1	3577	11	NULL	NULL	0	NULL	collagenase	Protein	neutrophil	binds to 					collagen	Protein				NULL		0	NULL	NULL	NULL	gw60_infectimmun_67_5_2319_s_233	10225890	(B) Analysis of active and latent forms of neutrophil collagenase binding to collagen.	bind
8105	1	3578	6	11	NULL	NULL	NULL	GCNF	GP		bind					Nanog 	GP		DR0 sequence		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8507_s_251	16166633	(B) Analysis of binding of GCNF to the  Nanog DR0 sequence by EMSA.	bind
11262	1	3578	7	11	NULL	NULL	NULL	GCNF	GP		bind					Nanog	GP		DR0 sequence		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8507_s_251	16166633	(B) Analysis of binding of GCNF to the  Nanog DR0 sequence by EMSA.	bind
80887	1	3578	11	NULL	NULL	NULL	NULL	GCNF	Protein		binds to 					Nanog DR0 sequence	NucleicAcidSubstance				NULL	by EMSA	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8507_s_251	16166633	(B) Analysis of binding of GCNF to the  Nanog DR0 sequence by EMSA.	bind
8106	1	3579	6	11	NULL	NULL	NULL	Spt20p	GP		bind					HXT genes	GP				NULL	mot1- 1 mutant strain	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_4863_s_173	15923605	(B) Analysis of Spt20p binding to  HXT genes in a  mot1- 1 mutant strain after a shift to low glucose.	bind
11265	1	3579	7	11	NULL	NULL	NULL	Spt20p	GP		bind					HXT genes	GP				NULL	 mot1- 1 mutant strain	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_4863_s_173	15923605	(B) Analysis of Spt20p binding to  HXT genes in a  mot1- 1 mutant strain after a shift to low glucose.	bind
80888	1	3579	11	NULL	NULL	0	NULL	Spt20p	Protein		binds to 					HXT gene	Gene				NULL	mot1- 1 mutant strain	0	NULL	NULL	NULL	gw70_molcellbiol_25_12_4863_s_173	15923605	(B) Analysis of Spt20p binding to  HXT genes in a  mot1- 1 mutant strain after a shift to low glucose.	bind
8108	1	3580	6	11	NULL	NULL	NULL	nuclear cyclin T	GP		bind					Tat protein	GP	HIV-1;; wild type			NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_104	9491887	(B) Analysis of the binding of nuclear cyclin T and CDK9  to wild-type and activation domain mutant HIV-1 and HIV-2 Tat proteins.	bind
8109	2	3580	6	11	NULL	NULL	NULL	nuclear cyclin T	GP		bind					Tat protein	GP	HIV-1;; mutant	activation domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_104	9491887	(B) Analysis of the binding of nuclear cyclin T and CDK9  to wild-type and activation domain mutant HIV-1 and HIV-2 Tat proteins.	bind
8110	3	3580	6	11	NULL	NULL	NULL	nuclear cyclin T	GP		bind					Tat protein	GP	HIV-2;; wild type			NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_104	9491887	(B) Analysis of the binding of nuclear cyclin T and CDK9  to wild-type and activation domain mutant HIV-1 and HIV-2 Tat proteins.	bind
8111	4	3580	6	11	NULL	NULL	NULL	nuclear cyclin T	GP		bind					Tat protein	GP	 HIV-2;; mutant 	activation domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_104	9491887	(B) Analysis of the binding of nuclear cyclin T and CDK9  to wild-type and activation domain mutant HIV-1 and HIV-2 Tat proteins.	bind
8112	5	3580	6	11	NULL	NULL	NULL	CDK9	GP		bind					Tat protein	GP	HIV-1;; wild type			NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_104	9491887	(B) Analysis of the binding of nuclear cyclin T and CDK9  to wild-type and activation domain mutant HIV-1 and HIV-2 Tat proteins.	bind
8113	6	3580	6	11	NULL	NULL	NULL	CDK9	GP		bind					Tat protein	GP	HIV-1;; mutant	activation domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_104	9491887	(B) Analysis of the binding of nuclear cyclin T and CDK9  to wild-type and activation domain mutant HIV-1 and HIV-2 Tat proteins.	bind
8114	7	3580	6	11	NULL	NULL	NULL	CDK9	GP		bind					Tat protein	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_104	9491887	(B) Analysis of the binding of nuclear cyclin T and CDK9  to wild-type and activation domain mutant HIV-1 and HIV-2 Tat proteins.	bind
8115	8	3580	6	11	NULL	NULL	NULL	CDK9	GP		bind					Tat protein	GP	HIV-2;; mutant	activation domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_104	9491887	(B) Analysis of the binding of nuclear cyclin T and CDK9  to wild-type and activation domain mutant HIV-1 and HIV-2 Tat proteins.	bind
11269	1	3580	7	11	NULL	NULL	NULL	nuclear cyclin T	GP		bind					Tat protein	GP	wild-type;; HIV-1			NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_104	9491887	(B) Analysis of the binding of nuclear cyclin T and CDK9  to wild-type and activation domain mutant HIV-1 and HIV-2 Tat proteins.	bind
11271	2	3580	7	11	NULL	NULL	NULL	nuclear cyclin T	GP		bind					Tat protein	GP	wild-type;; HIV-2 			NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_104	9491887	(B) Analysis of the binding of nuclear cyclin T and CDK9  to wild-type and activation domain mutant HIV-1 and HIV-2 Tat proteins.	bind
11273	3	3580	7	11	NULL	NULL	NULL	nuclear cyclin T	GP		bind					Tat protein	GP	mutant;; HIV-1 	activation domain 		NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_104	9491887	(B) Analysis of the binding of nuclear cyclin T and CDK9  to wild-type and activation domain mutant HIV-1 and HIV-2 Tat proteins.	bind
11276	4	3580	7	11	NULL	NULL	NULL	nuclear cyclin T	GP		bind					Tat protein	GP	mutant;; HIV-2	activation domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_104	9491887	(B) Analysis of the binding of nuclear cyclin T and CDK9  to wild-type and activation domain mutant HIV-1 and HIV-2 Tat proteins.	bind
11279	5	3580	7	11	NULL	NULL	NULL	CDK9	GP		bind					Tat protein	GP	wild-type;; HIV-1			NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_104	9491887	(B) Analysis of the binding of nuclear cyclin T and CDK9  to wild-type and activation domain mutant HIV-1 and HIV-2 Tat proteins.	bind
11281	6	3580	7	11	NULL	NULL	NULL	CDK9	GP		bind					Tat protein	GP	wild-type;; HIV-2			NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_104	9491887	(B) Analysis of the binding of nuclear cyclin T and CDK9  to wild-type and activation domain mutant HIV-1 and HIV-2 Tat proteins.	bind
11283	7	3580	7	11	NULL	NULL	NULL	CDK9	GP		bind					Tat protein	GP	HIV-1;; mutant	activation domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_104	9491887	(B) Analysis of the binding of nuclear cyclin T and CDK9  to wild-type and activation domain mutant HIV-1 and HIV-2 Tat proteins.	bind
11289	8	3580	7	11	NULL	NULL	NULL	CDK9	GP		bind					Tat protein	GP	HIV-2;; mutant	activation domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_104	9491887	(B) Analysis of the binding of nuclear cyclin T and CDK9  to wild-type and activation domain mutant HIV-1 and HIV-2 Tat proteins.	bind
80889	1	3580	11	NULL	NULL	0	NULL	cyclin T	Protein	nuclear	binds to 					Tat protein	Protein	 wild-type;HIV-1			NULL		0	NULL	NULL	NULL	gw60_cell_92_4_451_s_104	9491887	(B) Analysis of the binding of nuclear cyclin T and CDK9  to wild-type and activation domain mutant HIV-1 and HIV-2 Tat proteins.	bind
80890	2	3580	11	NULL	NULL	0	NULL	cyclin T	Protein	nuclear	binds to 					Tat protein	Protein	wild-type;;HIV-2			NULL		0	NULL	NULL	NULL	gw60_cell_92_4_451_s_104	9491887	(B) Analysis of the binding of nuclear cyclin T and CDK9  to wild-type and activation domain mutant HIV-1 and HIV-2 Tat proteins.	bind
80891	3	3580	11	NULL	NULL	0	NULL	cyclin T	Protein	nuclear	binds to 					Tat protein	Protein	HIV-1	activation domain mutant 		NULL		0	NULL	NULL	NULL	gw60_cell_92_4_451_s_104	9491887	(B) Analysis of the binding of nuclear cyclin T and CDK9  to wild-type and activation domain mutant HIV-1 and HIV-2 Tat proteins.	bind
80892	4	3580	11	NULL	NULL	0	NULL	cyclin T	Protein	nuclear	binds to 					Tat protein	Protein	 HIV-2	activation domain mutant		NULL		0	NULL	NULL	NULL	gw60_cell_92_4_451_s_104	9491887	(B) Analysis of the binding of nuclear cyclin T and CDK9  to wild-type and activation domain mutant HIV-1 and HIV-2 Tat proteins.	bind
80893	5	3580	11	NULL	NULL	0	NULL	CDK9	Protein	nuclear	binds to 					Tat protein	Protein	wild-type;HIV-1			NULL		0	NULL	NULL	NULL	gw60_cell_92_4_451_s_104	9491887	(B) Analysis of the binding of nuclear cyclin T and CDK9  to wild-type and activation domain mutant HIV-1 and HIV-2 Tat proteins.	bind
80894	6	3580	11	NULL	NULL	NULL	NULL	CDK9	Protein	nuclear	binds to 					Tat protein	Protein	wild-type;;HIV-2			NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_104	9491887	(B) Analysis of the binding of nuclear cyclin T and CDK9  to wild-type and activation domain mutant HIV-1 and HIV-2 Tat proteins.	bind
80895	7	3580	11	NULL	NULL	0	NULL	CDK9	Protein	nuclear	binds to 					Tat protein	Protein	HIV-1	activation domain mutant		NULL		0	NULL	NULL	NULL	gw60_cell_92_4_451_s_104	9491887	(B) Analysis of the binding of nuclear cyclin T and CDK9  to wild-type and activation domain mutant HIV-1 and HIV-2 Tat proteins.	bind
80896	8	3580	11	NULL	NULL	NULL	NULL	CDK9	Protein	nuclear	binds to 					Tat protein	Protein	HIV-2	activation domain mutant		NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_104	9491887	(B) Analysis of the binding of nuclear cyclin T and CDK9  to wild-type and activation domain mutant HIV-1 and HIV-2 Tat proteins.	bind
8116	1	3582	6	11	NULL	NULL	NULL	GST-PBD	GP		bind					small G proteins	GP	transfected			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_971_s_234	11238453	(B) Analysis of the effects of PSGAP on GST-PBD or GST-RBD binding to transfected small G proteins.	bind
8117	2	3582	6	11	NULL	NULL	NULL	GST-RBD	GP		bind					small G proteins	GP	transfected			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_971_s_234	11238453	(B) Analysis of the effects of PSGAP on GST-PBD or GST-RBD binding to transfected small G proteins.	bind
11299	1	3582	7	11	NULL	NULL	NULL	GST-PBD	GP		bind					small G protein	GP	transfected			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_971_s_234	11238453	(B) Analysis of the effects of PSGAP on GST-PBD or GST-RBD binding to transfected small G proteins.	bind
11301	2	3582	7	11	NULL	NULL	NULL	GST-RBD	GP		bind					small G protein	GP	transfected			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_971_s_234	11238453	(B) Analysis of the effects of PSGAP on GST-PBD or GST-RBD binding to transfected small G proteins.	bind
80897	1	3582	11	NULL	NULL	0	NULL	GST-PBD	Protein		binds to 					small G protein	Protein	transfected			NULL		0	NULL	NULL	NULL	gw60_cellbiol_152_5_971_s_234	11238453	(B) Analysis of the effects of PSGAP on GST-PBD or GST-RBD binding to transfected small G proteins.	bind
80898	2	3582	11	NULL	NULL	0	NULL	GST-RBD	Protein		binds to 					small G protein	Protein	transfected			NULL		0	NULL	NULL	NULL	gw60_cellbiol_152_5_971_s_234	11238453	(B) Analysis of the effects of PSGAP on GST-PBD or GST-RBD binding to transfected small G proteins.	bind
8118	1	3583	6	11	NULL	NULL	NULL	Bm	GP		bind					BLMA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2311_s_292	11706014	(B) and the type II'' beta-turn from Arg43A to Ile46A exhibit large conformational changes due to the binding of Bm to BLMA (Fig.  5,  a and  b).	bind
8119	2	3583	6	11	NULL	NULL	NULL	statement 1	Process		changes					Arg43A	AminoAcid	conformation of 	type II'' beta-turn		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2311_s_292	11706014	(B) and the type II'' beta-turn from Arg43A to Ile46A exhibit large conformational changes due to the binding of Bm to BLMA (Fig.  5,  a and  b).	bind
8120	3	3583	6	11	NULL	NULL	NULL	statement 1	Process		changes					Ile46A	AminoAcid	conformation of 	type II'' beta-turn		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2311_s_292	11706014	(B) and the type II'' beta-turn from Arg43A to Ile46A exhibit large conformational changes due to the binding of Bm to BLMA (Fig.  5,  a and  b).	bind
11307	1	3583	7	11	NULL	NULL	NULL	Bm	GP		bind					BLMA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2311_s_292	11706014	(B) and the type II'' beta-turn from Arg43A to Ile46A exhibit large conformational changes due to the binding of Bm to BLMA (Fig.  5,  a and  b).	bind
11313	2	3583	7	11	NULL	NULL	NULL	statement 1	Process		change					type II'' beta-turn	AminoAcid	conformation of	Arg43A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2311_s_292	11706014	(B) and the type II'' beta-turn from Arg43A to Ile46A exhibit large conformational changes due to the binding of Bm to BLMA (Fig.  5,  a and  b).	bind
15047	3	3583	7	11	NULL	NULL	NULL	statement 1	Process		change					type II'' beta-turn	AminoAcid	conformation of	Ile46A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2311_s_292	11706014	(B) and the type II'' beta-turn from Arg43A to Ile46A exhibit large conformational changes due to the binding of Bm to BLMA (Fig.  5,  a and  b).	bind
80899	1	3583	11	NULL	NULL	0	NULL	Bm	Chemical		binds to 					BLMA	Protein				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_3_2311_s_292	11706014	(B) and the type II'' beta-turn from Arg43A to Ile46A exhibit large conformational changes due to the binding of Bm to BLMA (Fig.  5,  a and  b).	bind
8121	1	3584	6	11	NULL	NULL	NULL	p53	GP		bind					p300	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_1_s_361	16267266	(b) Another effect of ATM-induced p53 phosphorylation  is to stimulate the binding of p53 to p300 (which probably competes with Mdm2 for  p53 binding).	bind
8122	2	3584	6	11	NULL	NULL	NULL	ATM	GP		induces					p53	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_1_s_361	16267266	(b) Another effect of ATM-induced p53 phosphorylation  is to stimulate the binding of p53 to p300 (which probably competes with Mdm2 for  p53 binding).	bind
8123	3	3584	6	11	NULL	NULL	NULL	statement 2	Process		stimulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_1_s_361	16267266	(b) Another effect of ATM-induced p53 phosphorylation  is to stimulate the binding of p53 to p300 (which probably competes with Mdm2 for  p53 binding).	bind
8124	4	3584	6	11	NULL	NULL	NULL	Mdm2	GP		bind					p53	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_1_s_361	16267266	(b) Another effect of ATM-induced p53 phosphorylation  is to stimulate the binding of p53 to p300 (which probably competes with Mdm2 for  p53 binding).	bind
8125	5	3584	6	11	NULL	NULL	NULL	statement 1	Process		competes with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_1_s_361	16267266	(b) Another effect of ATM-induced p53 phosphorylation  is to stimulate the binding of p53 to p300 (which probably competes with Mdm2 for  p53 binding).	bind
11317	1	3584	7	11	NULL	NULL	NULL	 p53	GP		bind					p300	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_1_s_361	16267266	(b) Another effect of ATM-induced p53 phosphorylation  is to stimulate the binding of p53 to p300 (which probably competes with Mdm2 for  p53 binding).	bind
11319	2	3584	7	11	NULL	NULL	NULL	ATM	GP		induce					p53	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_1_s_361	16267266	(b) Another effect of ATM-induced p53 phosphorylation  is to stimulate the binding of p53 to p300 (which probably competes with Mdm2 for  p53 binding).	bind
11321	3	3584	7	11	NULL	NULL	NULL	statement 2	Process		stimulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_1_s_361	16267266	(b) Another effect of ATM-induced p53 phosphorylation  is to stimulate the binding of p53 to p300 (which probably competes with Mdm2 for  p53 binding).	bind
11322	4	3584	7	11	NULL	NULL	NULL	Mdm2	GP		bind					p53	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_1_s_361	16267266	(b) Another effect of ATM-induced p53 phosphorylation  is to stimulate the binding of p53 to p300 (which probably competes with Mdm2 for  p53 binding).	bind
11325	5	3584	7	11	NULL	NULL	NULL	statement 1	Process		compete with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_1_s_361	16267266	(b) Another effect of ATM-induced p53 phosphorylation  is to stimulate the binding of p53 to p300 (which probably competes with Mdm2 for  p53 binding).	bind
80903	1	3584	11	NULL	NULL	0	NULL	ATM	Protein		phosphorylate					p53	Protein				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_1_1_s_361	16267266	(b) Another effect of ATM-induced p53 phosphorylation  is to stimulate the binding of p53 to p300 (which probably competes with Mdm2 for  p53 binding).	bind
80904	2	3584	11	NULL	NULL	0	NULL	p53	Protein		binds to 					p300	Protein				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_1_1_s_361	16267266	(b) Another effect of ATM-induced p53 phosphorylation  is to stimulate the binding of p53 to p300 (which probably competes with Mdm2 for  p53 binding).	bind
80905	3	3584	11	NULL	NULL	0	NULL	statement 1	Process		stimulates					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_1_1_s_361	16267266	(b) Another effect of ATM-induced p53 phosphorylation  is to stimulate the binding of p53 to p300 (which probably competes with Mdm2 for  p53 binding).	bind
80906	4	3584	11	NULL	NULL	0	NULL	Mdm2	Protein		binds to 					p53	Protein				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_1_1_s_361	16267266	(b) Another effect of ATM-induced p53 phosphorylation  is to stimulate the binding of p53 to p300 (which probably competes with Mdm2 for  p53 binding).	bind
80907	5	3584	11	NULL	NULL	0	NULL	statement 2	Process		competes with					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_1_1_s_361	16267266	(b) Another effect of ATM-induced p53 phosphorylation  is to stimulate the binding of p53 to p300 (which probably competes with Mdm2 for  p53 binding).	bind
8126	1	3585	6	11	NULL	NULL	NULL	transactivator	GP	positive	bind					P2 sequence	NucleicAcid				NULL	BCL1 nuclear extract	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_284_s_252	9858552	(B) Anti-CDP pre- and postincubation using 1 mug of a nuclear extract from a B-cell line (BCL1) that lacks NF-muNR but contains a positive transactivator (Bright) that binds the same P2 sequence.	bind
8127	2	3585	6	11	NULL	NULL	NULL	BCL1	GP		is a type of					B-cell line	Cell				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_284_s_252	9858552	(B) Anti-CDP pre- and postincubation using 1 mug of a nuclear extract from a B-cell line (BCL1) that lacks NF-muNR but contains a positive transactivator (Bright) that binds the same P2 sequence.	bind
11329	1	3585	7	11	NULL	NULL	NULL	transactivator	GP	positive	bind					P2 sequence	NucleicAcid				NULL	BCL1 nuclear extract	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_284_s_252	9858552	(B) Anti-CDP pre- and postincubation using 1 mug of a nuclear extract from a B-cell line (BCL1) that lacks NF-muNR but contains a positive transactivator (Bright) that binds the same P2 sequence.	bind
44766	2	3585	7	11	NULL	NULL	NULL	BCL1	GP		is a type of					B-cell line	Cell				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_284_s_252	9858552	(B) Anti-CDP pre- and postincubation using 1 mug of a nuclear extract from a B-cell line (BCL1) that lacks NF-muNR but contains a positive transactivator (Bright) that binds the same P2 sequence.	bind
80908	1	3585	11	NULL	NULL	0	NULL	positive transactivator	GeneOrProtein		binds to 					P2 sequence	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_1_284_s_252	9858552	(B) Anti-CDP pre- and postincubation using 1 mug of a nuclear extract from a B-cell line (BCL1) that lacks NF-muNR but contains a positive transactivator (Bright) that binds the same P2 sequence.	bind
8128	1	3588	6	11	NULL	NULL	NULL	Anti-mCD100 	GP		bind		specifically			CD100-CHO cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_immunity_13_5_621_s_54	11114375	(B) Anti-mCD100 mAb binds specifically to CD100-CHO cells.	bind
40784	2	3588	6	11	NULL	NULL	NULL	Anti-mCD100	GP		is a type of					monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_13_5_621_s_54	11114375	(B) Anti-mCD100 mAb binds specifically to CD100-CHO cells.	bind
11762	1	3588	7	11	NULL	NULL	NULL	Anti-mCD100 mAb	GP		bind		specifically			CD100-CHO cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_immunity_13_5_621_s_54	11114375	(B) Anti-mCD100 mAb binds specifically to CD100-CHO cells.	bind
44767	2	3588	7	11	NULL	NULL	NULL	Anti-mCD100	GP		is a type of					monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_13_5_621_s_54	11114375	(B) Anti-mCD100 mAb binds specifically to CD100-CHO cells.	bind
80909	1	3588	11	NULL	NULL	0	NULL	Anti-mCD100 mAb	PartOfProtein		binds to 		specifically			CD100-CHO cells	Cell				NULL		0	NULL	NULL	NULL	gw60_immunity_13_5_621_s_54	11114375	(B) Anti-mCD100 mAb binds specifically to CD100-CHO cells.	bind
8129	1	3589	6	11	NULL	NULL	NULL	myosin-Va	GP		bind					syntaxin-1A	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_281	16030255	(B) Anti-myosin-V neck antiserum inhibits the binding of myosin-Va by syntaxin-1A.	bind
8130	2	3589	6	11	NULL	NULL	NULL	Anti-myosin-V	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_281	16030255	(B) Anti-myosin-V neck antiserum inhibits the binding of myosin-Va by syntaxin-1A.	bind
40785	3	3589	6	11	NULL	NULL	NULL	Anti-myosin-V	GP		is a type of					neck antiserum	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_281	16030255	(B) Anti-myosin-V neck antiserum inhibits the binding of myosin-Va by syntaxin-1A.	bind
11763	1	3589	7	11	NULL	NULL	NULL	myosin-Va	GP		bind					syntaxin-1A	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_281	16030255	(B) Anti-myosin-V neck antiserum inhibits the binding of myosin-Va by syntaxin-1A.	bind
11764	2	3589	7	11	NULL	NULL	NULL	Anti-myosin-V 	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_281	16030255	(B) Anti-myosin-V neck antiserum inhibits the binding of myosin-Va by syntaxin-1A.	bind
44769	3	3589	7	11	NULL	NULL	NULL	Anti-myosin-V	GP		is a type of					neck antiserum	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_281	16030255	(B) Anti-myosin-V neck antiserum inhibits the binding of myosin-Va by syntaxin-1A.	bind
80910	1	3589	11	NULL	NULL	0	NULL	myosin-Va	Protein		binds to 					syntaxin-1A	Protein				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_281	16030255	(B) Anti-myosin-V neck antiserum inhibits the binding of myosin-Va by syntaxin-1A.	bind
80911	2	3589	11	NULL	NULL	0	NULL	Anti-myosin-V	PartOfProtein	neck antiserum	inhibits					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_281	16030255	(B) Anti-myosin-V neck antiserum inhibits the binding of myosin-Va by syntaxin-1A.	bind
8131	1	3590	6	11	NULL	NULL	NULL	Asf1p	GP		bind					Cac2p	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_2_614_s_214	11756556	(B) Asf1p binds Cac2p in vitro.	bind
11765	1	3590	7	11	NULL	NULL	NULL	Asf1p	GP		binds					Cac2p	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_2_614_s_214	11756556	(B) Asf1p binds Cac2p in vitro.	bind
80912	1	3590	11	NULL	NULL	0	NULL	Asf1p	Protein		binds to 					Cac2p	Protein				NULL	in vitro	0	NULL	NULL	NULL	gw60_molcellbiol_22_2_614_s_214	11756556	(B) Asf1p binds Cac2p in vitro.	bind
8132	1	3591	6	11	NULL	NULL	NULL	GST-myogenin	GP		bind					MEF-1 oligodeoxynucleotide	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_1074_s_278	9448005	(B) Assays involving the binding of GST-myogenin fusion protein to the MEF-1 oligodeoxynucleotide.	bind
40787	2	3591	6	11	NULL	NULL	NULL	GST-myogenin	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_1074_s_278	9448005	(B) Assays involving the binding of GST-myogenin fusion protein to the MEF-1 oligodeoxynucleotide.	bind
11766	1	3591	7	11	NULL	NULL	NULL	GST-myogenin	GP		binds					MEF-1 oligodeoxynucleotide	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_1074_s_278	9448005	(B) Assays involving the binding of GST-myogenin fusion protein to the MEF-1 oligodeoxynucleotide.	bind
80913	1	3591	11	NULL	NULL	0	NULL	GST-myogenin fusion protein	Protein		binds to 					MEF-1 oligodeoxynucleotide	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_2_1074_s_278	9448005	(B) Assays involving the binding of GST-myogenin fusion protein to the MEF-1 oligodeoxynucleotide.	bind
80914	1	3592	11	NULL	NULL	0	NULL	TRAF4	Protein	knockdown	phosphorylate		serine			p47phox	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_6_2320_s_258	15743827	(B) Assessment of serine  phosphorylation of p47phox after knockdown of TRAF4.	bind
8133	1	3593	6	11	NULL	NULL	NULL	PAK4	GP	endogenous	bind					integrin beta5	GP		membrane-proximal region within cytoplasmic domain		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_158_7_1287_s_75	12356872	(B) Association of endogenous PAK4 with the membrane-proximal region within integrin beta5 cytoplasmic domain was examined by a GST pull-down assay, including GST fused to a beta5 deletion mutant lacking the PAK4-binding region mapped by yeast two-hybrid analysis.	bind
11768	1	3593	7	11	NULL	NULL	NULL	PAK4	GP	endogenous	bind					integrin beta5 	GP		membrane-proximal region within cytoplasmic domain		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_158_7_1287_s_75	12356872	(B) Association of endogenous PAK4 with the membrane-proximal region within integrin beta5 cytoplasmic domain was examined by a GST pull-down assay, including GST fused to a beta5 deletion mutant lacking the PAK4-binding region mapped by yeast two-hybrid analysis.	bind
80915	1	3593	11	NULL	NULL	NULL	NULL	PAK4	Protein	endogenous	associated with					integrin beta5	Protein	membrane-proximal region	cytoplasmic domain		NULL	GST pull-down assay	NULL	NULL	NULL	NULL	gw60_cellbiol_158_7_1287_s_75	12356872	(B) Association of endogenous PAK4 with the membrane-proximal region within integrin beta5 cytoplasmic domain was examined by a GST pull-down assay, including GST fused to a beta5 deletion mutant lacking the PAK4-binding region mapped by yeast two-hybrid analysis.	bind
80916	2	3593	11	NULL	NULL	0	NULL	GST	Protein		fused to					beta5 deletion mutant	Protein	lacking the PAK4-binding region			NULL	yeast two-hybrid analysis	0	NULL	NULL	NULL	gw60_cellbiol_158_7_1287_s_75	12356872	(B) Association of endogenous PAK4 with the membrane-proximal region within integrin beta5 cytoplasmic domain was examined by a GST pull-down assay, including GST fused to a beta5 deletion mutant lacking the PAK4-binding region mapped by yeast two-hybrid analysis.	bind
8134	1	3594	6	11	NULL	NULL	NULL	p85alpha subunit	GP		bind					p110alpha	GP				NULL	NIH 3T3 cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7119_s_144	9819398	(B) Association of p85alpha subunit with p110alpha and p110beta in NIH 3T3 cells.	bind
8135	2	3594	6	11	NULL	NULL	NULL	p85alpha subunit	GP		bind					p110beta	GP				NULL	NIH 3T3 cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7119_s_144	9819398	(B) Association of p85alpha subunit with p110alpha and p110beta in NIH 3T3 cells.	bind
11769	1	3594	7	11	NULL	NULL	NULL	p85 alpha subunit	GP		bind					p110alpha	GP				NULL	NIH 3T3 cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7119_s_144	9819398	(B) Association of p85alpha subunit with p110alpha and p110beta in NIH 3T3 cells.	bind
11770	2	3594	7	11	NULL	NULL	NULL	p85 alpha subunit	GP		bind					p110beta	GP				NULL	NIH 3T3 cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7119_s_144	9819398	(B) Association of p85alpha subunit with p110alpha and p110beta in NIH 3T3 cells.	bind
80917	1	3594	11	NULL	NULL	NULL	NULL	p85alpha	Protein		associated with					 p110alpha	Protein				NULL	in NIH 3T3 cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7119_s_144	9819398	(B) Association of p85alpha subunit with p110alpha and p110beta in NIH 3T3 cells.	bind
80918	2	3594	11	NULL	NULL	0	NULL	p85alpha	Protein		associated with					p110beta	Protein				NULL	in NIH 3T3 cells	0	NULL	NULL	NULL	gw60_molcellbiol_18_12_7119_s_144	9819398	(B) Association of p85alpha subunit with p110alpha and p110beta in NIH 3T3 cells.	bind
8136	1	3595	6	11	NULL	NULL	NULL	Stat3	GP		associates with					Etk	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2043_s_174	10688651	(B) Association of STAT3 with Etk or its deletion mutants.	bind
8137	2	3595	6	11	NULL	NULL	NULL	Stat3	GP		associates with					Etk	GP	deletion mutants			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2043_s_174	10688651	(B) Association of STAT3 with Etk or its deletion mutants.	bind
8138	3	3595	6	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2043_s_174	10688651	(B) Association of STAT3 with Etk or its deletion mutants.	bind
11771	1	3595	7	11	NULL	NULL	NULL	STAT3	GP		associates with					Etk	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2043_s_174	10688651	(B) Association of STAT3 with Etk or its deletion mutants.	bind
11772	2	3595	7	11	NULL	NULL	NULL	STAT3	GP		associates with					Etk	GP	deletion mutant			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2043_s_174	10688651	(B) Association of STAT3 with Etk or its deletion mutants.	bind
15048	3	3595	7	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2043_s_174	10688651	(B) Association of STAT3 with Etk or its deletion mutants.	bind
80919	1	3595	11	NULL	NULL	0	NULL	STAT3	Protein		associated with					 Etk 	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_6_2043_s_174	10688651	(B) Association of STAT3 with Etk or its deletion mutants.	bind
80920	2	3595	11	NULL	NULL	0	NULL	STAT3	Protein		associated with					Etk	Protein	deletion mutant			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_6_2043_s_174	10688651	(B) Association of STAT3 with Etk or its deletion mutants.	bind
80921	3	3595	11	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_6_2043_s_174	10688651	(B) Association of STAT3 with Etk or its deletion mutants.	bind
8139	1	3596	6	11	NULL	NULL	NULL	ATP	Chemical		bind					TAP1	GP				NULL	wild type transporter	NULL	NULL	NULL	NULL	gw60_currbiol_11_4_242_s_67	11250152	(b) ATP binding capacity of TAP1 and TAP2 in wild-type transporter.	bind
8140	2	3596	6	11	NULL	NULL	NULL	ATP	Chemical		bind					TAP2	GP				NULL	wild type transporter	NULL	NULL	NULL	NULL	gw60_currbiol_11_4_242_s_67	11250152	(b) ATP binding capacity of TAP1 and TAP2 in wild-type transporter.	bind
11773	1	3596	7	11	NULL	NULL	NULL	TAP1	GP		bind					ATP	Chemical				NULL	wild-type transporter	NULL	NULL	NULL	NULL	gw60_currbiol_11_4_242_s_67	11250152	(b) ATP binding capacity of TAP1 and TAP2 in wild-type transporter.	bind
11774	2	3596	7	11	NULL	NULL	NULL	TAP2	GP		bind					ATP	Chemical				NULL	wild-type transporter	NULL	NULL	NULL	NULL	gw60_currbiol_11_4_242_s_67	11250152	(b) ATP binding capacity of TAP1 and TAP2 in wild-type transporter.	bind
80922	1	3596	11	NULL	NULL	0	NULL	ATP	Chemical		binds to 					TAP1	Protein	in wild-type transporter			NULL		0	NULL	NULL	NULL	gw60_currbiol_11_4_242_s_67	11250152	(b) ATP binding capacity of TAP1 and TAP2 in wild-type transporter.	bind
80923	2	3596	11	NULL	NULL	0	NULL	ATP	Protein		binds to 					TAP2	Protein	in wild-type transporter			NULL		0	NULL	NULL	NULL	gw60_currbiol_11_4_242_s_67	11250152	(b) ATP binding capacity of TAP1 and TAP2 in wild-type transporter.	bind
8141	1	3598	6	11	NULL	NULL	NULL	ATP	Chemical		bind					GroEL	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_869_s_29	11779463	(b) ATP binding to GroEL alters  its conformation, weakens the binding of substrate, and permits  the binding of GroES to the ATP-bound  ring.	bind
8142	2	3598	6	11	NULL	NULL	NULL	statement 1	Process		alters					GroEL	GP	conformation of 			NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_869_s_29	11779463	(b) ATP binding to GroEL alters  its conformation, weakens the binding of substrate, and permits  the binding of GroES to the ATP-bound  ring.	bind
8143	3	3598	6	11	NULL	NULL	NULL	statement 1	Process		weakens					substrate	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_869_s_29	11779463	(b) ATP binding to GroEL alters  its conformation, weakens the binding of substrate, and permits  the binding of GroES to the ATP-bound  ring.	bind
8144	4	3598	6	11	NULL	NULL	NULL	ATP	Chemical		bind					ring	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_869_s_29	11779463	(b) ATP binding to GroEL alters  its conformation, weakens the binding of substrate, and permits  the binding of GroES to the ATP-bound  ring.	bind
8145	5	3598	6	11	NULL	NULL	NULL	GroES	GP		bind					statement 4	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_869_s_29	11779463	(b) ATP binding to GroEL alters  its conformation, weakens the binding of substrate, and permits  the binding of GroES to the ATP-bound  ring.	bind
8146	6	3598	6	11	NULL	NULL	NULL	statement 1	Process		permits					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_869_s_29	11779463	(b) ATP binding to GroEL alters  its conformation, weakens the binding of substrate, and permits  the binding of GroES to the ATP-bound  ring.	bind
11775	1	3598	7	11	NULL	NULL	NULL	ATP	Chemical		binds to					GroEL	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_869_s_29	11779463	(b) ATP binding to GroEL alters  its conformation, weakens the binding of substrate, and permits  the binding of GroES to the ATP-bound  ring.	bind
11776	2	3598	7	11	NULL	NULL	NULL	statement 1	Process		alters					GroEL	GP	conformation of			NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_869_s_29	11779463	(b) ATP binding to GroEL alters  its conformation, weakens the binding of substrate, and permits  the binding of GroES to the ATP-bound  ring.	bind
11777	3	3598	7	11	NULL	NULL	NULL	statement 1	Process		weakens 					substrate	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_869_s_29	11779463	(b) ATP binding to GroEL alters  its conformation, weakens the binding of substrate, and permits  the binding of GroES to the ATP-bound  ring.	bind
11778	4	3598	7	11	NULL	NULL	NULL	GroES	GP		bind					statement 6	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_869_s_29	11779463	(b) ATP binding to GroEL alters  its conformation, weakens the binding of substrate, and permits  the binding of GroES to the ATP-bound  ring.	bind
11779	5	3598	7	11	NULL	NULL	NULL	statement 1	Process		permits					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_869_s_29	11779463	(b) ATP binding to GroEL alters  its conformation, weakens the binding of substrate, and permits  the binding of GroES to the ATP-bound  ring.	bind
52995	6	3598	7	11	NULL	NULL	NULL	ATP	Chemical		bind					ring	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_869_s_29	11779463	(b) ATP binding to GroEL alters  its conformation, weakens the binding of substrate, and permits  the binding of GroES to the ATP-bound  ring.	bind
80924	1	3598	11	NULL	NULL	0	NULL	ATP	Chemical		binds to 					GroEL	Protein				NULL		0	NULL	NULL	NULL	gw60_cell_107_7_869_s_29	11779463	(b) ATP binding to GroEL alters  its conformation, weakens the binding of substrate, and permits  the binding of GroES to the ATP-bound  ring.	bind
80925	2	3598	11	NULL	NULL	0	NULL	statement 1	Process		alters					conformation	Process	GroEL			NULL		0	NULL	NULL	NULL	gw60_cell_107_7_869_s_29	11779463	(b) ATP binding to GroEL alters  its conformation, weakens the binding of substrate, and permits  the binding of GroES to the ATP-bound  ring.	bind
80926	3	3598	11	NULL	NULL	0	NULL	statement 1	Process		weakens					binding	BiologicalProcess	substrate			NULL		0	NULL	NULL	NULL	gw60_cell_107_7_869_s_29	11779463	(b) ATP binding to GroEL alters  its conformation, weakens the binding of substrate, and permits  the binding of GroES to the ATP-bound  ring.	bind
80927	4	3598	11	NULL	NULL	0	NULL	GroES 	Protein		binds to 					ATP-bound ring	Chemical				NULL		0	NULL	NULL	NULL	gw60_cell_107_7_869_s_29	11779463	(b) ATP binding to GroEL alters  its conformation, weakens the binding of substrate, and permits  the binding of GroES to the ATP-bound  ring.	bind
80928	5	3598	11	NULL	NULL	0	NULL	statement 1	Process		permits					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_cell_107_7_869_s_29	11779463	(b) ATP binding to GroEL alters  its conformation, weakens the binding of substrate, and permits  the binding of GroES to the ATP-bound  ring.	bind
80929	1	3599	11	NULL	NULL	0	NULL	HisP	Protein	binding pocket	binds to 					ATP	Chemical				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1561_1_47_s_82	11988180	(B) ATP-binding pocket of HisP.	bind
8154	1	3602	6	11	NULL	NULL	NULL	Dam1p	GP	in vitro-translated	bind					Ndc80 complex-associated beads	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_8_3342_s_230	12925767	(B) Bar graph shows the percentage of IVT  Dam1p bound to Ndc80 complex-associated beads.	bind
11781	1	3602	7	11	NULL	NULL	NULL	Dam1p	GP	in vitro-translated	bind					Ndc80 complex-associated beads	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_8_3342_s_230	12925767	(B) Bar graph shows the percentage of IVT  Dam1p bound to Ndc80 complex-associated beads.	bind
80930	1	3602	11	NULL	NULL	0	NULL	Ndc80 complex	Protein		associated with					beads	Chemical				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_8_3342_s_230	12925767	(B) Bar graph shows the percentage of IVT  Dam1p bound to Ndc80 complex-associated beads.	bind
80931	2	3602	11	NULL	NULL	0	NULL	Dam1p	Protein	IVT	binds to 					statement 1	Chemical				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_8_3342_s_230	12925767	(B) Bar graph shows the percentage of IVT  Dam1p bound to Ndc80 complex-associated beads.	bind
8155	1	3603	6	11	NULL	NULL	NULL	PP1	GP		bind		weakly			Cdc25	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_4_1779_s_263	16467385	(B) Based on data presented here, we speculate that PP1 binds  weakly to Cdc25 and inefficient dephosphorylation of S287 is allowed after 14-3-3  removal.	bind
11782	1	3603	7	11	NULL	NULL	NULL	PP1	GP		binds		weakly			Cdc25	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_4_1779_s_263	16467385	(B) Based on data presented here, we speculate that PP1 binds  weakly to Cdc25 and inefficient dephosphorylation of S287 is allowed after 14-3-3  removal.	bind
80932	1	3603	11	NULL	NULL	0	NULL	PP1	Protein		binds to 		weakly			Cdc25	Protein				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_4_1779_s_263	16467385	(B) Based on data presented here, we speculate that PP1 binds  weakly to Cdc25 and inefficient dephosphorylation of S287 is allowed after 14-3-3  removal.	bind
80933	2	3603	11	NULL	NULL	0	NULL	14-3-3	Protein		removed from					Cdc25	Protein				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_4_1779_s_263	16467385	(B) Based on data presented here, we speculate that PP1 binds  weakly to Cdc25 and inefficient dephosphorylation of S287 is allowed after 14-3-3  removal.	bind
80934	3	3603	11	NULL	NULL	0	NULL	PP1	Protein		dephosphorylate		inefficiently			S287	Protein				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_4_1779_s_263	16467385	(B) Based on data presented here, we speculate that PP1 binds  weakly to Cdc25 and inefficient dephosphorylation of S287 is allowed after 14-3-3  removal.	bind
80935	4	3603	11	NULL	NULL	0	NULL	statement 3	Process		occurs after					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_4_1779_s_263	16467385	(B) Based on data presented here, we speculate that PP1 binds  weakly to Cdc25 and inefficient dephosphorylation of S287 is allowed after 14-3-3  removal.	bind
80936	1	3604	11	NULL	NULL	0	NULL	beta-galactosidase	Protein		is					beta-gal	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_19_7214_s_92	10982838	(B) beta-Galactosidase activity of  sec61-2 mutant cells carrying plasmids expressing beta-galactosidase (beta-gal), the beta-galactosidase-SL17 fusion protein (beta-gal-SL17) ( 11), or beta-galactosidase with an N-terminal lysine residue (K-beta-gal) ( 2) at permissive and nonpermissive temperatures.	bind
80937	2	3604	11	NULL	NULL	0	NULL	beta-gal-SL17	Protein		is					beta-galactosidase-SL17 fusion protein	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_19_7214_s_92	10982838	(B) beta-Galactosidase activity of  sec61-2 mutant cells carrying plasmids expressing beta-galactosidase (beta-gal), the beta-galactosidase-SL17 fusion protein (beta-gal-SL17) ( 11), or beta-galactosidase with an N-terminal lysine residue (K-beta-gal) ( 2) at permissive and nonpermissive temperatures.	bind
80938	3	3604	11	NULL	NULL	0	NULL	beta-galactosidase	Protein		is			N-terminal lysine residue		K-beta-gal	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_19_7214_s_92	10982838	(B) beta-Galactosidase activity of  sec61-2 mutant cells carrying plasmids expressing beta-galactosidase (beta-gal), the beta-galactosidase-SL17 fusion protein (beta-gal-SL17) ( 11), or beta-galactosidase with an N-terminal lysine residue (K-beta-gal) ( 2) at permissive and nonpermissive temperatures.	bind
80939	4	3604	11	NULL	NULL	0	NULL	sec61-2 mutant cells	cell		carrying					plasmid	NucleicAcidSubstance	beta-galactosidase			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_19_7214_s_92	10982838	(B) beta-Galactosidase activity of  sec61-2 mutant cells carrying plasmids expressing beta-galactosidase (beta-gal), the beta-galactosidase-SL17 fusion protein (beta-gal-SL17) ( 11), or beta-galactosidase with an N-terminal lysine residue (K-beta-gal) ( 2) at permissive and nonpermissive temperatures.	bind
80940	5	3604	11	NULL	NULL	0	NULL	sec61-2 mutant cells	cell		carrying					plasmid	NucleicAcidSubstance	beta-galactosidase-SL17 fusion protein			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_19_7214_s_92	10982838	(B) beta-Galactosidase activity of  sec61-2 mutant cells carrying plasmids expressing beta-galactosidase (beta-gal), the beta-galactosidase-SL17 fusion protein (beta-gal-SL17) ( 11), or beta-galactosidase with an N-terminal lysine residue (K-beta-gal) ( 2) at permissive and nonpermissive temperatures.	bind
80941	6	3604	11	NULL	NULL	0	NULL	sec61-2 mutant cells	cell		carrying					plasmid	NucleicAcidSubstance	K-beta-gal			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_19_7214_s_92	10982838	(B) beta-Galactosidase activity of  sec61-2 mutant cells carrying plasmids expressing beta-galactosidase (beta-gal), the beta-galactosidase-SL17 fusion protein (beta-gal-SL17) ( 11), or beta-galactosidase with an N-terminal lysine residue (K-beta-gal) ( 2) at permissive and nonpermissive temperatures.	bind
8156	1	3605	6	11	NULL	NULL	NULL	 3[H]QNB	Chemical		bind					mAChR	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainres_950_1_10_s_179	12231224	(B) Bilirubin protects 3[H]QNB binding to the mAChR from inhibition by 2  M heme and 100  M hydrogen peroxide.	bind
8157	2	3605	6	11	NULL	NULL	NULL	heme	Chemical		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_brainres_950_1_10_s_179	12231224	(B) Bilirubin protects 3[H]QNB binding to the mAChR from inhibition by 2  M heme and 100  M hydrogen peroxide.	bind
8158	3	3605	6	11	NULL	NULL	NULL	hydrogen peroxide	Chemical		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_brainres_950_1_10_s_179	12231224	(B) Bilirubin protects 3[H]QNB binding to the mAChR from inhibition by 2  M heme and 100  M hydrogen peroxide.	bind
8159	4	3605	6	11	NULL	NULL	NULL	Bilirubin	Chemical		protects					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_brainres_950_1_10_s_179	12231224	(B) Bilirubin protects 3[H]QNB binding to the mAChR from inhibition by 2  M heme and 100  M hydrogen peroxide.	bind
8160	5	3605	6	11	NULL	NULL	NULL	Bilirubin	Chemical		protects					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_brainres_950_1_10_s_179	12231224	(B) Bilirubin protects 3[H]QNB binding to the mAChR from inhibition by 2  M heme and 100  M hydrogen peroxide.	bind
11795	1	3605	7	11	NULL	NULL	NULL	3[H]QNB	Chemical		bind					mAChR	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainres_950_1_10_s_179	12231224	(B) Bilirubin protects 3[H]QNB binding to the mAChR from inhibition by 2  M heme and 100  M hydrogen peroxide.	bind
11796	2	3605	7	11	NULL	NULL	NULL	statement 1	Process		is inhibited by					heme	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_brainres_950_1_10_s_179	12231224	(B) Bilirubin protects 3[H]QNB binding to the mAChR from inhibition by 2  M heme and 100  M hydrogen peroxide.	bind
11797	3	3605	7	11	NULL	NULL	NULL	statement 1	Process		is inhibited by					hydrogen peroxide	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_brainres_950_1_10_s_179	12231224	(B) Bilirubin protects 3[H]QNB binding to the mAChR from inhibition by 2  M heme and 100  M hydrogen peroxide.	bind
11798	4	3605	7	11	NULL	NULL	NULL	Bilirubin	Chemical		protects					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_brainres_950_1_10_s_179	12231224	(B) Bilirubin protects 3[H]QNB binding to the mAChR from inhibition by 2  M heme and 100  M hydrogen peroxide.	bind
11799	5	3605	7	11	NULL	NULL	NULL	Bilirubin	Chemical		protects					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_brainres_950_1_10_s_179	12231224	(B) Bilirubin protects 3[H]QNB binding to the mAChR from inhibition by 2  M heme and 100  M hydrogen peroxide.	bind
80942	1	3605	11	NULL	NULL	0	NULL	3[H]QNB	Chemical		binds to 					mAChR	Protein				NULL		0	NULL	NULL	NULL	gw60_brainres_950_1_10_s_179	12231224	(B) Bilirubin protects 3[H]QNB binding to the mAChR from inhibition by 2  M heme and 100  M hydrogen peroxide.	bind
80943	2	3605	11	NULL	NULL	0	NULL	heme	Protein		inhibits					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_brainres_950_1_10_s_179	12231224	(B) Bilirubin protects 3[H]QNB binding to the mAChR from inhibition by 2  M heme and 100  M hydrogen peroxide.	bind
80944	3	3605	11	NULL	NULL	0	NULL	hydrogen peroxide	Chemical		inhibits					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_brainres_950_1_10_s_179	12231224	(B) Bilirubin protects 3[H]QNB binding to the mAChR from inhibition by 2  M heme and 100  M hydrogen peroxide.	bind
80945	4	3605	11	NULL	NULL	0	NULL	Bilirubin	Chemical		prevents					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_brainres_950_1_10_s_179	12231224	(B) Bilirubin protects 3[H]QNB binding to the mAChR from inhibition by 2  M heme and 100  M hydrogen peroxide.	bind
80946	5	3605	11	NULL	NULL	0	NULL	Bilirubin	Chemical		prevents					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_brainres_950_1_10_s_179	12231224	(B) Bilirubin protects 3[H]QNB binding to the mAChR from inhibition by 2  M heme and 100  M hydrogen peroxide.	bind
8161	1	3607	6	11	NULL	NULL	NULL	peptide ligands	GP		bind					Mena	GP		EVH1 domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_97_4_471_s_63	10338211	(B) Binding affinities of  peptide ligands to Mena EVH1 domain measured by fluorescence perturbation. '''	bind
11801	1	3607	7	11	NULL	NULL	NULL	peptide ligands	GP		bind					Mena	GP		EVH1		NULL		NULL	NULL	NULL	NULL	gw60_cell_97_4_471_s_63	10338211	(B) Binding affinities of  peptide ligands to Mena EVH1 domain measured by fluorescence perturbation. '''	bind
80947	1	3607	11	NULL	NULL	0	NULL	peptide ligands	Chemical		binds to 					Mena EVH1 domain	PartOfProtein				NULL	fluorescence perturbation	0	NULL	NULL	NULL	gw60_cell_97_4_471_s_63	10338211	(B) Binding affinities of  peptide ligands to Mena EVH1 domain measured by fluorescence perturbation. '''	bind
40847	1	3608	6	11	NULL	NULL	NULL	Rab9	GP		bind					TIP47	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_12_5420_s_259	15456905	(B) Binding affinity of Rab9 and TIP47.	bind
11802	1	3608	7	11	NULL	NULL	NULL	Rab9	GP		bind					TIP47	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_12_5420_s_259	15456905	(B) Binding affinity of Rab9 and TIP47.	bind
80948	1	3608	11	NULL	NULL	0	NULL	Rab9	Protein		has affinity for					binding	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_12_5420_s_259	15456905	(B) Binding affinity of Rab9 and TIP47.	bind
80949	2	3608	11	NULL	NULL	0	NULL	TIP47	Protein		has affinity for					binding	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_12_5420_s_259	15456905	(B) Binding affinity of Rab9 and TIP47.	bind
8162	1	3609	6	11	NULL	NULL	NULL	APP	GP		bind			C-terminus		KLC1	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_28_2_449_s_131	11144355	(B) Binding analysis of APP C terminus to KLC1.	bind
11803	1	3609	7	11	NULL	NULL	NULL	 APP 	GP		bind			C terminus		KLC1	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_28_2_449_s_131	11144355	(B) Binding analysis of APP C terminus to KLC1.	bind
80950	1	3609	11	NULL	NULL	0	NULL	APP	Protein	C terminus	binds to 					KLC1	Protein				NULL		0	NULL	NULL	NULL	gw60_neuron_28_2_449_s_131	11144355	(B) Binding analysis of APP C terminus to KLC1.	bind
80951	1	3614	11	NULL	NULL	NULL	NULL	ER	CellComponent		binds to 					p300	Protein				NULL	mammalian one-hybrid system	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_312_3_656_s_90	14680815	(B) Binding between ER  and p300  was examined using the mammalian one-hybrid system.	bind
8165	1	3615	6	11	NULL	NULL	NULL	p110alpha PI3-K	GP		bind					R-Ras	GP	mutant	effector loop		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_6333_s_212	10454580	(B) Binding between p110alpha PI3-K and different R-Ras effector loop mutants was evaluated by an in vitro pull-down assay.	bind
52996	1	3615	7	11	NULL	NULL	NULL	p110alpha PI3-K	GP		bind					R-Ras	GP	mutant	effector loop		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_6333_s_212	10454580	(B) Binding between p110alpha PI3-K and different R-Ras effector loop mutants was evaluated by an in vitro pull-down assay.	bind
80952	1	3615	11	NULL	NULL	0	NULL	PI3-K	Protein		binds to 			p110alpha		R-Ras effector loop mutants	Protein				NULL	in vitro pull-down assay	0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6333_s_212	10454580	(B) Binding between p110alpha PI3-K and different R-Ras effector loop mutants was evaluated by an in vitro pull-down assay.	bind
8166	1	3616	6	11	NULL	NULL	NULL	PALA	AminoAcid		bind					ATCase	GP		active site		NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_65_3_404_s_90	11528003	(B) Binding mode of the bisubstrate analogue PALA (purple) to the active site of  ATCase.	bind
40866	2	3616	6	11	NULL	NULL	NULL	PALA	AminoAcid		is a type of					bisubstrate analogue	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_65_3_404_s_90	11528003	(B) Binding mode of the bisubstrate analogue PALA (purple) to the active site of  ATCase.	bind
11807	1	3616	7	11	NULL	NULL	NULL	PALA	AminoAcid		bind					ATCase	GP		active site of		NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_65_3_404_s_90	11528003	(B) Binding mode of the bisubstrate analogue PALA (purple) to the active site of  ATCase.	bind
44770	2	3616	7	11	NULL	NULL	NULL	PALA	AminoAcid		is a type of					bisubstrate analogue	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_65_3_404_s_90	11528003	(B) Binding mode of the bisubstrate analogue PALA (purple) to the active site of  ATCase.	bind
80953	1	3616	11	NULL	NULL	0	NULL	 PALA	Chemical	bisubstrate analogue	binds to 					ATCase	Protein	active site			NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_65_3_404_s_90	11528003	(B) Binding mode of the bisubstrate analogue PALA (purple) to the active site of  ATCase.	bind
8167	1	3618	6	11	NULL	NULL	NULL	VASP	GP	purified	bind					M10	GP		tail		NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_319_1_214_s_80	15158464	(B) Binding of  purified VASP and M10 tail.	bind
11808	1	3618	7	11	NULL	NULL	NULL	VASP	GP	purified	bind					M10	GP		tail		NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_319_1_214_s_80	15158464	(B) Binding of  purified VASP and M10 tail.	bind
80954	1	3618	11	NULL	NULL	0	NULL	VASP	Protein	purified	binds to 					M10 tail	Protein				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_319_1_214_s_80	15158464	(B) Binding of  purified VASP and M10 tail.	bind
8168	1	3619	6	11	NULL	NULL	NULL	UFD2	GP	recombinant	bind					Ubi-GST	GP	ubiquitinated			NULL		NULL	NULL	NULL	NULL	gw60_cell_96_5_635_s_78	10089879	(B) Binding of  recombinant UFD2 to ubiquitinated Ubi-GST.	bind
11809	1	3619	7	11	NULL	NULL	NULL	UFD2	GP	recombinant	bind					Ubi-GST	GP	ubiquitinated			NULL		NULL	NULL	NULL	NULL	gw60_cell_96_5_635_s_78	10089879	(B) Binding of  recombinant UFD2 to ubiquitinated Ubi-GST.	bind
80955	1	3619	11	NULL	NULL	0	NULL	UFD2	Protein	recombinant	binds to 					Ubi-GST	Protein	ubiquitinated			NULL		0	NULL	NULL	NULL	gw60_cell_96_5_635_s_78	10089879	(B) Binding of  recombinant UFD2 to ubiquitinated Ubi-GST.	bind
8169	1	3620	6	11	NULL	NULL	NULL	eIF-4E	GP		bind					m7-GTP-Sepharose resin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_6041_s_119	10454551	(B) Binding of 4BP-1 to eIF-4E (already bound to m7-GTP-Sepharose resin) was determined.	bind
8170	2	3620	6	11	NULL	NULL	NULL	4BP-1	GP		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_6041_s_119	10454551	(B) Binding of 4BP-1 to eIF-4E (already bound to m7-GTP-Sepharose resin) was determined.	bind
11810	1	3620	7	11	NULL	NULL	NULL	eIF-4E	GP		bind					m7-GTP-Sepharose resin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_6041_s_119	10454551	(B) Binding of 4BP-1 to eIF-4E (already bound to m7-GTP-Sepharose resin) was determined.	bind
15049	2	3620	7	11	NULL	NULL	NULL	4BP-1	GP		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_6041_s_119	10454551	(B) Binding of 4BP-1 to eIF-4E (already bound to m7-GTP-Sepharose resin) was determined.	bind
80956	1	3620	11	NULL	NULL	0	NULL	4BP-1	Protein		binds to 					eIF-4E	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6041_s_119	10454551	(B) Binding of 4BP-1 to eIF-4E (already bound to m7-GTP-Sepharose resin) was determined.	bind
80957	2	3620	11	NULL	NULL	0	NULL	eIF-4E	Protein		binds to 					m7-GTP-Sepharose resin	Chemical				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6041_s_119	10454551	(B) Binding of 4BP-1 to eIF-4E (already bound to m7-GTP-Sepharose resin) was determined.	bind
8171	1	3621	6	11	NULL	NULL	NULL	CstF-64	GP		bind			RNA-BD		pA1 transcript	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_10_2_261_s_159	10072078	(B) Binding of a GST-RNA binding domain protein (-RNA BD) of CstF-64 to pA1 and pA2 transcripts.	bind
8172	2	3621	6	11	NULL	NULL	NULL	CstF-64	GP		bind			RNA-BD		pA2 transcript	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_10_2_261_s_159	10072078	(B) Binding of a GST-RNA binding domain protein (-RNA BD) of CstF-64 to pA1 and pA2 transcripts.	bind
8173	3	3621	6	11	NULL	NULL	NULL	RNA BD	GP		is					RNA binding domain	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_10_2_261_s_159	10072078	(B) Binding of a GST-RNA binding domain protein (-RNA BD) of CstF-64 to pA1 and pA2 transcripts.	bind
11811	1	3621	7	11	NULL	NULL	NULL	 CstF-64	GP		bind			RNA BD		pA1 transcript	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_10_2_261_s_159	10072078	(B) Binding of a GST-RNA binding domain protein (-RNA BD) of CstF-64 to pA1 and pA2 transcripts.	bind
11812	2	3621	7	11	NULL	NULL	NULL	CstF-64	GP		bind			RNA BD		pA2 transcript	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_10_2_261_s_159	10072078	(B) Binding of a GST-RNA binding domain protein (-RNA BD) of CstF-64 to pA1 and pA2 transcripts.	bind
11813	3	3621	7	11	NULL	NULL	NULL	RNA BD	GP		is					RNA binding domain	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_10_2_261_s_159	10072078	(B) Binding of a GST-RNA binding domain protein (-RNA BD) of CstF-64 to pA1 and pA2 transcripts.	bind
80958	1	3621	11	NULL	NULL	0	NULL	CstF-64	Protein		binds to 			GST-RNA binding domain		pA1	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_immunity_10_2_261_s_159	10072078	(B) Binding of a GST-RNA binding domain protein (-RNA BD) of CstF-64 to pA1 and pA2 transcripts.	bind
80959	2	3621	11	NULL	NULL	0	NULL	CstF-64	Protein		binds to 			GST-RNA binding domain		pA2	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_immunity_10_2_261_s_159	10072078	(B) Binding of a GST-RNA binding domain protein (-RNA BD) of CstF-64 to pA1 and pA2 transcripts.	bind
8193	1	3622	6	11	NULL	NULL	NULL	NES	GP		bind					CRM1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_22_7862_s_163	11604520	(B) Binding of a NES to CRM1 occurs in a tripartite complex with RanGTP.	bind
8370	2	3622	6	11	NULL	NULL	NULL	statement 1	GP		bind					RanGTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_22_7862_s_163	11604520	(B) Binding of a NES to CRM1 occurs in a tripartite complex with RanGTP.	bind
8371	3	3622	6	11	NULL	NULL	NULL	statement 2	Process		forms					tripartite complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_22_7862_s_163	11604520	(B) Binding of a NES to CRM1 occurs in a tripartite complex with RanGTP.	bind
11814	1	3622	7	11	NULL	NULL	NULL	NES	GP		bind					CRM1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_22_7862_s_163	11604520	(B) Binding of a NES to CRM1 occurs in a tripartite complex with RanGTP.	bind
11815	2	3622	7	11	NULL	NULL	NULL	statement 1	GP		bind					RanGTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_22_7862_s_163	11604520	(B) Binding of a NES to CRM1 occurs in a tripartite complex with RanGTP.	bind
11816	3	3622	7	11	NULL	NULL	NULL	statement 2	Process		forms					tripartite complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_22_7862_s_163	11604520	(B) Binding of a NES to CRM1 occurs in a tripartite complex with RanGTP.	bind
80960	1	3622	11	NULL	NULL	0	NULL	NES	Chemical		binds to 					CRM1	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_22_7862_s_163	11604520	(B) Binding of a NES to CRM1 occurs in a tripartite complex with RanGTP.	bind
80961	2	3622	11	NULL	NULL	0	NULL	statement 1	Protein		complex with 		tripartite			RanGTP	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_22_7862_s_163	11604520	(B) Binding of a NES to CRM1 occurs in a tripartite complex with RanGTP.	bind
8229	1	3624	6	11	NULL	NULL	NULL	biotin	Chemical		bind			RGD		uPAR - alpha5beta1 - Fn complexes	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_3_501_s_156	15684035	(B) Binding of biotin-RGD to uPAR - alpha5beta1 - Fn complexes.	bind
11817	1	3624	7	11	NULL	NULL	NULL	biotin	Chemical		bind			RGD		uPAR - alpha5beta1 - Fn complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_3_501_s_156	15684035	(B) Binding of biotin-RGD to uPAR - alpha5beta1 - Fn complexes.	bind
80962	1	3624	11	NULL	NULL	0	NULL	uPAR	Protein		binds to 					alpha5beta1	Protein				NULL		0	NULL	NULL	NULL	gw70_cellbiol_168_3_501_s_156	15684035	(B) Binding of biotin-RGD to uPAR - alpha5beta1 - Fn complexes.	bind
80963	2	3624	11	NULL	NULL	0	NULL	statement 1	Protein		complex with 					Fn	Protein				NULL		0	NULL	NULL	NULL	gw70_cellbiol_168_3_501_s_156	15684035	(B) Binding of biotin-RGD to uPAR - alpha5beta1 - Fn complexes.	bind
80964	3	3624	11	NULL	NULL	0	NULL	statement 2	Protein		binds to 					biotin-RGD	Chemical				NULL		0	NULL	NULL	NULL	gw70_cellbiol_168_3_501_s_156	15684035	(B) Binding of biotin-RGD to uPAR - alpha5beta1 - Fn complexes.	bind
8230	1	3625	6	11	NULL	NULL	NULL	C/EBP-beta	GP	purified	bind					K15	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_8_3168_s_263	15060141	(B) Binding of C/EBP-beta to the K15 promoter  region by gel shift analysis with the purified CEB/Pbeta protein and the -266/-353  probe.	bind
11818	1	3625	7	11	NULL	NULL	NULL	C/EBP-beta	GP	purified	bind					K15	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_8_3168_s_263	15060141	(B) Binding of C/EBP-beta to the K15 promoter  region by gel shift analysis with the purified CEB/Pbeta protein and the -266/-353  probe.	bind
81009	1	3625	11	NULL	NULL	0	NULL	C/EBP-beta	Protein		binds to 					K15 promoter	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_8_3168_s_263	15060141	(B) Binding of C/EBP-beta to the K15 promoter  region by gel shift analysis with the purified CEB/Pbeta protein and the -266/-353  probe.	bind
8231	1	3626	6	11	NULL	NULL	NULL	C/EBPbeta	GP		bind					p40	GP	endogenous		promoter	NULL	bone marrow-derived macrophages	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_6_2385_s_205	14993278	(B) Binding of C/EBPbeta to the endogenous p40 promoter was monitored by ChIP and  semiquantitative PCR by using C/EBPbeta antibodies and chromatin samples prepared  from bone marrow-derived macrophages.	bind
11819	1	3626	7	11	NULL	NULL	NULL	C/EBPbeta	GP		bind					p40	GP	endogenous		promoter	NULL	bone marrow-derived macrophages	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_6_2385_s_205	14993278	(B) Binding of C/EBPbeta to the endogenous p40 promoter was monitored by ChIP and  semiquantitative PCR by using C/EBPbeta antibodies and chromatin samples prepared  from bone marrow-derived macrophages.	bind
81010	1	3626	11	NULL	NULL	0	NULL	C/EBPbeta	Protein		binds to 					p40 promoter 	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_6_2385_s_205	14993278	(B) Binding of C/EBPbeta to the endogenous p40 promoter was monitored by ChIP and  semiquantitative PCR by using C/EBPbeta antibodies and chromatin samples prepared  from bone marrow-derived macrophages.	bind
8232	1	3627	6	11	NULL	NULL	NULL	CCR5 antisera	GP		bind					CCR5 receptor transfectants	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_2_112_s_51	9024623	(b) Binding of CCR5 antisera to CCR5 receptor transfectants.	bind
11820	1	3627	7	11	NULL	NULL	NULL	CCR5 antisera	GP		bind					CCR5 receptor transfectant	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_2_112_s_51	9024623	(b) Binding of CCR5 antisera to CCR5 receptor transfectants.	bind
81011	1	3627	11	NULL	NULL	0	NULL	CCR5 antisera	PartOfProtein		binds to 					CCR5 receptor transfectants	Cell				NULL		0	NULL	NULL	NULL	gw60_currbiol_7_2_112_s_51	9024623	(b) Binding of CCR5 antisera to CCR5 receptor transfectants.	bind
8233	1	3628	6	11	NULL	NULL	NULL	Cdc20 fragments	GP		bind					CCT	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_87_s_247	12887895	(B) Binding of Cdc20 fragments to the CCT, the APC/C, and Mad2.	bind
8234	2	3628	6	11	NULL	NULL	NULL	Cdc20 fragments	GP		bind					APC/C	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_87_s_247	12887895	(B) Binding of Cdc20 fragments to the CCT, the APC/C, and Mad2.	bind
8235	3	3628	6	11	NULL	NULL	NULL	Cdc20 fragments	GP		bind					Mad2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_87_s_247	12887895	(B) Binding of Cdc20 fragments to the CCT, the APC/C, and Mad2.	bind
11821	1	3628	7	11	NULL	NULL	NULL	 Cdc20 fragments	GP		bind					CCT	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_87_s_247	12887895	(B) Binding of Cdc20 fragments to the CCT, the APC/C, and Mad2.	bind
11822	2	3628	7	11	NULL	NULL	NULL	Cdc20 fragments	GP		bind					APC/C	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_87_s_247	12887895	(B) Binding of Cdc20 fragments to the CCT, the APC/C, and Mad2.	bind
11823	3	3628	7	11	NULL	NULL	NULL	Cdc20 fragments	GP		bind		  			Mad2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_87_s_247	12887895	(B) Binding of Cdc20 fragments to the CCT, the APC/C, and Mad2.	bind
81012	1	3628	11	NULL	NULL	0	NULL	Cdc20 fragment	PartOfProtein		binds to 					CCT	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcell_12_1_87_s_247	12887895	(B) Binding of Cdc20 fragments to the CCT, the APC/C, and Mad2.	bind
81013	2	3628	11	NULL	NULL	0	NULL	Cdc20 fragment	PartOfProtein		binds to 					APC/C	Protein				NULL		0	NULL	NULL	NULL	gw60_molcell_12_1_87_s_247	12887895	(B) Binding of Cdc20 fragments to the CCT, the APC/C, and Mad2.	bind
81014	3	3628	11	NULL	NULL	0	NULL	Cdc20 fragment	PartOfProtein		binds to 					Mad2	Protein				NULL		0	NULL	NULL	NULL	gw60_molcell_12_1_87_s_247	12887895	(B) Binding of Cdc20 fragments to the CCT, the APC/C, and Mad2.	bind
8236	1	3629	6	11	NULL	NULL	NULL	CIDR1alpha	GP		bind					IgG	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_9_5412_s_163	15322039	(B) Binding of CIDR1alpha to IgG of different species.	bind
11824	1	3629	7	11	NULL	NULL	NULL	 CIDR1alpha	GP		bind					IgG	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_9_5412_s_163	15322039	(B) Binding of CIDR1alpha to IgG of different species.	bind
81015	1	3629	11	NULL	NULL	0	NULL	CIDR1alpha	Protein		binds to 					IgG	PartOfProtein				NULL		0	NULL	NULL	NULL	gw70_infectimmun_72_9_5412_s_163	15322039	(B) Binding of CIDR1alpha to IgG of different species.	bind
8237	1	3630	6	11	NULL	NULL	NULL	CksHs2	GP		bind					p33 cdk2	GP	monomeric			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_3659_s_221	9632748	(B) Binding of CksHs2 to monomeric p33 cdk2.	bind
11825	1	3630	7	11	NULL	NULL	NULL	CksHs2	GP		bind					p33 cdk2	GP	monomeric			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_3659_s_221	9632748	(B) Binding of CksHs2 to monomeric p33 cdk2.	bind
81016	1	3630	11	NULL	NULL	0	NULL	CksHs2	Protein		binds to 					p33 cdk2	Protein	monomeric			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_7_3659_s_221	9632748	(B) Binding of CksHs2 to monomeric p33 cdk2.	bind
8238	1	3631	6	11	NULL	NULL	NULL	cyclin A	GP		bind					Skp2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_635_s_220	9858587	(B) Binding of cyclin A and cyclin E to Skp2.	bind
8239	2	3631	6	11	NULL	NULL	NULL	Cyclin E	GP		bind					Skp2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_635_s_220	9858587	(B) Binding of cyclin A and cyclin E to Skp2.	bind
11826	1	3631	7	11	NULL	NULL	NULL	cyclin A	GP		bind					Skp2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_635_s_220	9858587	(B) Binding of cyclin A and cyclin E to Skp2.	bind
11827	2	3631	7	11	NULL	NULL	NULL	cyclin E	GP		bind					Skp2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_635_s_220	9858587	(B) Binding of cyclin A and cyclin E to Skp2.	bind
81017	1	3631	11	NULL	NULL	0	NULL	cyclin A	Protein		binds to 					Skp2	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_1_635_s_220	9858587	(B) Binding of cyclin A and cyclin E to Skp2.	bind
81018	2	3631	11	NULL	NULL	0	NULL	cyclin E	Protein		binds to 					Skp2	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_1_635_s_220	9858587	(B) Binding of cyclin A and cyclin E to Skp2.	bind
8240	1	3632	6	11	NULL	NULL	NULL	Dbl	GP		bind					Rho proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_11_7870_s_271	10523675	(B) Binding of Dbl to Rho proteins.	bind
11828	1	3632	7	11	NULL	NULL	NULL	Dbl	GP		bind					Rho protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_11_7870_s_271	10523675	(B) Binding of Dbl to Rho proteins.	bind
81019	1	3632	11	NULL	NULL	0	NULL	Dbl	Protein		binds to 					Rho protein	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_11_7870_s_271	10523675	(B) Binding of Dbl to Rho proteins.	bind
8241	1	3633	6	11	NULL	NULL	NULL	Nef alleles	GP		bind					V1H	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_13_6_2045_s_112	12058068	(B) Binding of different Nef alleles and Nef mutants to V1H indicates that the integrity of the flexible loop structure is required for the interaction.	bind
8242	2	3633	6	11	NULL	NULL	NULL	Nef	GP	mutants	bind					V1H	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_13_6_2045_s_112	12058068	(B) Binding of different Nef alleles and Nef mutants to V1H indicates that the integrity of the flexible loop structure is required for the interaction.	bind
8243	3	3633	6	11	NULL	NULL	NULL	flexible loop structure	GP	integrity of	is required for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_13_6_2045_s_112	12058068	(B) Binding of different Nef alleles and Nef mutants to V1H indicates that the integrity of the flexible loop structure is required for the interaction.	bind
8244	4	3633	6	11	NULL	NULL	NULL	flexible loop structure	GP	integrity of	is required for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_13_6_2045_s_112	12058068	(B) Binding of different Nef alleles and Nef mutants to V1H indicates that the integrity of the flexible loop structure is required for the interaction.	bind
11829	1	3633	7	11	NULL	NULL	NULL	Nef alleles	GP		bind					V1H	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_13_6_2045_s_112	12058068	(B) Binding of different Nef alleles and Nef mutants to V1H indicates that the integrity of the flexible loop structure is required for the interaction.	bind
11830	2	3633	7	11	NULL	NULL	NULL	Nef 	GP	mutant	bind					V1H	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_13_6_2045_s_112	12058068	(B) Binding of different Nef alleles and Nef mutants to V1H indicates that the integrity of the flexible loop structure is required for the interaction.	bind
11831	3	3633	7	11	NULL	NULL	NULL	flexible loop structure	GP	integrity of	is required for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_13_6_2045_s_112	12058068	(B) Binding of different Nef alleles and Nef mutants to V1H indicates that the integrity of the flexible loop structure is required for the interaction.	bind
11832	4	3633	7	11	NULL	NULL	NULL	flexible loop structure	GP	integrity of	is required for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_13_6_2045_s_112	12058068	(B) Binding of different Nef alleles and Nef mutants to V1H indicates that the integrity of the flexible loop structure is required for the interaction.	bind
81020	1	3633	11	NULL	NULL	0	NULL	Nef allele	NucleicAcidSubstance		binds to 					V1H	PartOfProtein				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_13_6_2045_s_112	12058068	(B) Binding of different Nef alleles and Nef mutants to V1H indicates that the integrity of the flexible loop structure is required for the interaction.	bind
81021	2	3633	11	NULL	NULL	0	NULL	Nef mutants	Protein		binds to 					V1H	PartOfProtein				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_13_6_2045_s_112	12058068	(B) Binding of different Nef alleles and Nef mutants to V1H indicates that the integrity of the flexible loop structure is required for the interaction.	bind
8245	1	3634	6	11	NULL	NULL	NULL	dMyc	GP		bind					nnp-1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_9_3401_s_181	15831447	(B) Binding of dMyc to the  nnp-1 promoter.	bind
11833	1	3634	7	11	NULL	NULL	NULL	dMyc	GP		bind					nnp-1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_9_3401_s_181	15831447	(B) Binding of dMyc to the  nnp-1 promoter.	bind
81022	1	3634	11	NULL	NULL	0	NULL	dMyc	GeneOrProtein		binds to 					nnp-1 promoter	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_9_3401_s_181	15831447	(B) Binding of dMyc to the  nnp-1 promoter.	bind
8246	1	3635	6	11	NULL	NULL	NULL	DpiA protein	GP		bind					pSC101	GP			origin region	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_20_6025_s_72	14526013	(B) Binding of DpiA protein and the mutant proteins to the origin regions  of pSC101 and P1 are shown.	bind
8247	2	3635	6	11	NULL	NULL	NULL	DipA protein	GP	mutant	bind					P1	GP			origin region	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_20_6025_s_72	14526013	(B) Binding of DpiA protein and the mutant proteins to the origin regions  of pSC101 and P1 are shown.	bind
52997	3	3635	6	11	NULL	NULL	NULL	DpiA protein	GP		bind					P1	GP			origin region	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_20_6025_s_72	14526013	(B) Binding of DpiA protein and the mutant proteins to the origin regions  of pSC101 and P1 are shown.	bind
52998	4	3635	6	11	NULL	NULL	NULL	DpiA protein	GP	mutant	bind					pSC101	GP			origin region	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_20_6025_s_72	14526013	(B) Binding of DpiA protein and the mutant proteins to the origin regions  of pSC101 and P1 are shown.	bind
11834	1	3635	7	11	NULL	NULL	NULL	DpiA protein	GP		bind					pSC101	GP			origin region	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_20_6025_s_72	14526013	(B) Binding of DpiA protein and the mutant proteins to the origin regions  of pSC101 and P1 are shown.	bind
11835	2	3635	7	11	NULL	NULL	NULL	DpiA protein	GP		bind					P1	GP			origin region	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_20_6025_s_72	14526013	(B) Binding of DpiA protein and the mutant proteins to the origin regions  of pSC101 and P1 are shown.	bind
11836	3	3635	7	11	NULL	NULL	NULL	DpiA protein	GP	mutant	bind					pSC101	GP			origin region	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_20_6025_s_72	14526013	(B) Binding of DpiA protein and the mutant proteins to the origin regions  of pSC101 and P1 are shown.	bind
11837	4	3635	7	11	NULL	NULL	NULL	DpiA protein	GP	mutant	bind					P1	GP			origin region	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_20_6025_s_72	14526013	(B) Binding of DpiA protein and the mutant proteins to the origin regions  of pSC101 and P1 are shown.	bind
81023	1	3635	11	NULL	NULL	0	NULL	DpiA protein	Protein		binds to 					pSC101	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_20_6025_s_72	14526013	(B) Binding of DpiA protein and the mutant proteins to the origin regions  of pSC101 and P1 are shown.	bind
81024	2	3635	11	NULL	NULL	0	NULL	DpiA protein	Protein		binds to 					P1	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_20_6025_s_72	14526013	(B) Binding of DpiA protein and the mutant proteins to the origin regions  of pSC101 and P1 are shown.	bind
8248	1	3636	6	11	NULL	NULL	NULL	EF-Tu-GTP-aminoacyl-tRNA	NucleicAcid		bind					A/T (30S/50S)	NucleicAcid	hybrid state			NULL		NULL	NULL	NULL	NULL	gw60_structure_4_3_229_s_271	8805530	(b) Binding of EF-Tu-GTP-aminoacyl-tRNA to A/T (30S/50S) hybrid state.	bind
11838	1	3636	7	11	NULL	NULL	NULL	EF-Tu-GTP-aminoacyl-tRNA	NucleicAcid		bind					A/T (30S/50S)	NucleicAcid	hybrid state			NULL		NULL	NULL	NULL	NULL	gw60_structure_4_3_229_s_271	8805530	(b) Binding of EF-Tu-GTP-aminoacyl-tRNA to A/T (30S/50S) hybrid state.	bind
81025	1	3636	11	NULL	NULL	0	NULL	EF-Tu-GTP-aminoacyl-tRNA	NucleicAcidSubstance		binds to 					A/T	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_structure_4_3_229_s_271	8805530	(b) Binding of EF-Tu-GTP-aminoacyl-tRNA to A/T (30S/50S) hybrid state.	bind
8249	1	3637	6	11	NULL	NULL	NULL	eIF4G	GP		bind					Mnk2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_3_743_s_225	11154262	(B) Binding of eIF4G and ERK to Mnk2.	bind
8250	2	3637	6	11	NULL	NULL	NULL	ERK	GP		bind					Mnk2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_3_743_s_225	11154262	(B) Binding of eIF4G and ERK to Mnk2.	bind
11840	1	3637	7	11	NULL	NULL	NULL	eIF4G	GP		bind					Mnk2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_3_743_s_225	11154262	(B) Binding of eIF4G and ERK to Mnk2.	bind
11841	2	3637	7	11	NULL	NULL	NULL	ERK	GP		bind					Mnk2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_3_743_s_225	11154262	(B) Binding of eIF4G and ERK to Mnk2.	bind
81026	1	3637	11	NULL	NULL	0	NULL	eIF4G	Protein		binds to 					Mnk2	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_3_743_s_225	11154262	(B) Binding of eIF4G and ERK to Mnk2.	bind
81027	2	3637	11	NULL	NULL	0	NULL	ERK	Protein		binds to 					Mnk2	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_3_743_s_225	11154262	(B) Binding of eIF4G and ERK to Mnk2.	bind
8251	1	3638	6	11	NULL	NULL	NULL	eIF4G	GP		bind					Mnk1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_3_743_s_278	11154262	(B) Binding of eIF4G to Mnk1 and Mnk2 is reduced upon stimulation with phorbol ester.	bind
8252	2	3638	6	11	NULL	NULL	NULL	eIF4G	GP		bind					Mnk2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_3_743_s_278	11154262	(B) Binding of eIF4G to Mnk1 and Mnk2 is reduced upon stimulation with phorbol ester.	bind
8253	3	3638	6	11	NULL	NULL	NULL	statement 1	Process		reduced upon					phorbol ester	Chemical	stimulation with			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_3_743_s_278	11154262	(B) Binding of eIF4G to Mnk1 and Mnk2 is reduced upon stimulation with phorbol ester.	bind
8254	4	3638	6	11	NULL	NULL	NULL	statement 2	Process		reduced upon					phorbol ester	Chemical	stimulation with			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_3_743_s_278	11154262	(B) Binding of eIF4G to Mnk1 and Mnk2 is reduced upon stimulation with phorbol ester.	bind
11842	1	3638	7	11	NULL	NULL	NULL	eIF4G	GP		bind					Mnk1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_3_743_s_278	11154262	(B) Binding of eIF4G to Mnk1 and Mnk2 is reduced upon stimulation with phorbol ester.	bind
11843	2	3638	7	11	NULL	NULL	NULL	eIF4G	GP		bind					Mnk2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_3_743_s_278	11154262	(B) Binding of eIF4G to Mnk1 and Mnk2 is reduced upon stimulation with phorbol ester.	bind
11844	3	3638	7	11	NULL	NULL	NULL	statement 1	Process		is reduced upon					phorbol ester	Chemical	stimulation with			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_3_743_s_278	11154262	(B) Binding of eIF4G to Mnk1 and Mnk2 is reduced upon stimulation with phorbol ester.	bind
11845	4	3638	7	11	NULL	NULL	NULL	statement 2	Process		is reduced upon					phorbol ester	Chemical	stimulation with			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_3_743_s_278	11154262	(B) Binding of eIF4G to Mnk1 and Mnk2 is reduced upon stimulation with phorbol ester.	bind
81028	1	3638	11	NULL	NULL	0	NULL	eIF4G	Protein		binds to 					Mnk1	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_3_743_s_278	11154262	(B) Binding of eIF4G to Mnk1 and Mnk2 is reduced upon stimulation with phorbol ester.	bind
81029	2	3638	11	NULL	NULL	0	NULL	eIF4G	Protein		binds to 					Mnk2	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_3_743_s_278	11154262	(B) Binding of eIF4G to Mnk1 and Mnk2 is reduced upon stimulation with phorbol ester.	bind
81030	3	3638	11	NULL	NULL	0	NULL	 phorbol ester	Chemical		reduced					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_3_743_s_278	11154262	(B) Binding of eIF4G to Mnk1 and Mnk2 is reduced upon stimulation with phorbol ester.	bind
81031	4	3638	11	NULL	NULL	0	NULL	phorbol ester	Chemical		reduced					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_3_743_s_278	11154262	(B) Binding of eIF4G to Mnk1 and Mnk2 is reduced upon stimulation with phorbol ester.	bind
8255	1	3639	6	11	NULL	NULL	NULL	Rad24	GP		bind					Byr2	GP	FL			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_20_7105_s_264	12242289	(B) Binding of either Rad24 or Rad25 to Byr2FL, Byr2NT, and Byr2CT.	bind
8256	2	3639	6	11	NULL	NULL	NULL	Rad24	GP		bind					Byr2	GP		NT		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_20_7105_s_264	12242289	(B) Binding of either Rad24 or Rad25 to Byr2FL, Byr2NT, and Byr2CT.	bind
8257	3	3639	6	11	NULL	NULL	NULL	Rad24	GP		bind					Byr2	GP		CT		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_20_7105_s_264	12242289	(B) Binding of either Rad24 or Rad25 to Byr2FL, Byr2NT, and Byr2CT.	bind
8258	4	3639	6	11	NULL	NULL	NULL	Rad25	GP		bind					Byr2	GP	FL			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_20_7105_s_264	12242289	(B) Binding of either Rad24 or Rad25 to Byr2FL, Byr2NT, and Byr2CT.	bind
8259	5	3639	6	11	NULL	NULL	NULL	Rad25	GP		bind					Byr2	GP		NT		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_20_7105_s_264	12242289	(B) Binding of either Rad24 or Rad25 to Byr2FL, Byr2NT, and Byr2CT.	bind
8260	6	3639	6	11	NULL	NULL	NULL	Rad25	GP		bind					Byr2	GP		CT		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_20_7105_s_264	12242289	(B) Binding of either Rad24 or Rad25 to Byr2FL, Byr2NT, and Byr2CT.	bind
8261	7	3639	6	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_20_7105_s_264	12242289	(B) Binding of either Rad24 or Rad25 to Byr2FL, Byr2NT, and Byr2CT.	bind
8262	8	3639	6	11	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_20_7105_s_264	12242289	(B) Binding of either Rad24 or Rad25 to Byr2FL, Byr2NT, and Byr2CT.	bind
8263	9	3639	6	11	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_20_7105_s_264	12242289	(B) Binding of either Rad24 or Rad25 to Byr2FL, Byr2NT, and Byr2CT.	bind
11940	1	3639	7	11	NULL	NULL	NULL	Rad24	GP		bind					Byr2	GP	FL			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_20_7105_s_264	12242289	(B) Binding of either Rad24 or Rad25 to Byr2FL, Byr2NT, and Byr2CT.	bind
11941	2	3639	7	11	NULL	NULL	NULL	Rad24	GP		bind					Byr2	GP		NT		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_20_7105_s_264	12242289	(B) Binding of either Rad24 or Rad25 to Byr2FL, Byr2NT, and Byr2CT.	bind
11942	3	3639	7	11	NULL	NULL	NULL	Rad24	GP		bind					Byr2	GP		CT		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_20_7105_s_264	12242289	(B) Binding of either Rad24 or Rad25 to Byr2FL, Byr2NT, and Byr2CT.	bind
11943	4	3639	7	11	NULL	NULL	NULL	Rad25	GP		bind					Byr2	GP	FL			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_20_7105_s_264	12242289	(B) Binding of either Rad24 or Rad25 to Byr2FL, Byr2NT, and Byr2CT.	bind
11944	5	3639	7	11	NULL	NULL	NULL	Rad25	GP		bind					Byr2	GP		NT		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_20_7105_s_264	12242289	(B) Binding of either Rad24 or Rad25 to Byr2FL, Byr2NT, and Byr2CT.	bind
11945	6	3639	7	11	NULL	NULL	NULL	Rad25	GP		bind					Byr2	GP		CT		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_20_7105_s_264	12242289	(B) Binding of either Rad24 or Rad25 to Byr2FL, Byr2NT, and Byr2CT.	bind
53010	7	3639	7	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_20_7105_s_264	12242289	(B) Binding of either Rad24 or Rad25 to Byr2FL, Byr2NT, and Byr2CT.	bind
53011	8	3639	7	11	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_20_7105_s_264	12242289	(B) Binding of either Rad24 or Rad25 to Byr2FL, Byr2NT, and Byr2CT.	bind
53012	9	3639	7	11	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_20_7105_s_264	12242289	(B) Binding of either Rad24 or Rad25 to Byr2FL, Byr2NT, and Byr2CT.	bind
81032	1	3639	11	NULL	NULL	0	NULL	Rad24	Protein		binds to 					Byr2FL	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_20_7105_s_264	12242289	(B) Binding of either Rad24 or Rad25 to Byr2FL, Byr2NT, and Byr2CT.	bind
81033	2	3639	11	NULL	NULL	0	NULL	Rad24	Protein		binds to 					Byr2NT	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_20_7105_s_264	12242289	(B) Binding of either Rad24 or Rad25 to Byr2FL, Byr2NT, and Byr2CT.	bind
81034	3	3639	11	NULL	NULL	0	NULL	Rad24	Protein		binds to 					Byr2CT	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_20_7105_s_264	12242289	(B) Binding of either Rad24 or Rad25 to Byr2FL, Byr2NT, and Byr2CT.	bind
81035	4	3639	11	NULL	NULL	0	NULL	Rad25	Protein		binds to 					Byr2FL	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_20_7105_s_264	12242289	(B) Binding of either Rad24 or Rad25 to Byr2FL, Byr2NT, and Byr2CT.	bind
81036	5	3639	11	NULL	NULL	0	NULL	Rad25	Protein		binds to 					Byr2NT	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_20_7105_s_264	12242289	(B) Binding of either Rad24 or Rad25 to Byr2FL, Byr2NT, and Byr2CT.	bind
81037	6	3639	11	NULL	NULL	0	NULL	Rad25	Protein		binds to 					Byr2CT\t	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_20_7105_s_264	12242289	(B) Binding of either Rad24 or Rad25 to Byr2FL, Byr2NT, and Byr2CT.	bind
8264	1	3640	6	11	NULL	NULL	NULL	urokinase-type plasminogen activator	GP	exogenous	bind					BMEC	Cell	human			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_2_1014_s_175	15664945	(B) Binding of exogenous urokinase-type  plasminogen activator to human BMEC after spirochete addition.	bind
8265	2	3640	6	11	NULL	NULL	NULL	statement 1	Process		occurs after					spirochete	Organism	addition of			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_2_1014_s_175	15664945	(B) Binding of exogenous urokinase-type  plasminogen activator to human BMEC after spirochete addition.	bind
11946	1	3640	7	11	NULL	NULL	NULL	urokinase-type plasminogen activator	GP	exogenous	bind					BMEC	Cell	human			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_2_1014_s_175	15664945	(B) Binding of exogenous urokinase-type  plasminogen activator to human BMEC after spirochete addition.	bind
11947	2	3640	7	11	NULL	NULL	NULL	statement 1	Process		occurs after					spirochete	Organism	addition of			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_2_1014_s_175	15664945	(B) Binding of exogenous urokinase-type  plasminogen activator to human BMEC after spirochete addition.	bind
81038	1	3640	11	NULL	NULL	0	NULL	urokinase-type plasminogen activator	Protein	exogenous	binds to 					BMEC	Cell	human			NULL		0	NULL	NULL	NULL	gw70_infectimmun_73_2_1014_s_175	15664945	(B) Binding of exogenous urokinase-type  plasminogen activator to human BMEC after spirochete addition.	bind
81039	2	3640	11	NULL	NULL	0	NULL	spirochete	Organism		induces					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_infectimmun_73_2_1014_s_175	15664945	(B) Binding of exogenous urokinase-type  plasminogen activator to human BMEC after spirochete addition.	bind
8266	1	3641	6	11	NULL	NULL	NULL	fibrinogen	GP		bind					beta3 integrins	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_110_5_599_s_199	12230977	(B) Binding of fibrinogen to beta3 integrins.	bind
11948	1	3641	7	11	NULL	NULL	NULL	fibrinogen	GP		bind					beta3 integrins	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_110_5_599_s_199	12230977	(B) Binding of fibrinogen to beta3 integrins.	bind
81040	1	3641	11	NULL	NULL	0	NULL	fibrinogen	Protein		binds to 					beta3 integrin	Protein				NULL		0	NULL	NULL	NULL	gw60_cell_110_5_599_s_199	12230977	(B) Binding of fibrinogen to beta3 integrins.	bind
8267	1	3642	6	11	NULL	NULL	NULL	fibronectin	GP		bind					UspA1	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_9_4374_s_277	9712790	(B) Binding of fibronectin to UspA1.	bind
11949	1	3642	7	11	NULL	NULL	NULL	fibronectin	GP		bind					UspA1	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_9_4374_s_277	9712790	(B) Binding of fibronectin to UspA1.	bind
81041	1	3642	11	NULL	NULL	0	NULL	fibronectin	Protein		binds to 					UspA1	Protein				NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_9_4374_s_277	9712790	(B) Binding of fibronectin to UspA1.	bind
8268	1	3643	6	11	NULL	NULL	NULL	fip1-206	GP		bind					Pap1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_6_2026_s_328	11238938	(B) Binding of fip1-206 to Pap1 prevents specific polyadenylation.	bind
8269	2	3643	6	11	NULL	NULL	NULL	statement 1	Process		prevents					polyadenylation	Process	specific			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_6_2026_s_328	11238938	(B) Binding of fip1-206 to Pap1 prevents specific polyadenylation.	bind
11950	1	3643	7	11	NULL	NULL	NULL	fip1-206	GP		bind					Pap1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_6_2026_s_328	11238938	(B) Binding of fip1-206 to Pap1 prevents specific polyadenylation.	bind
11951	2	3643	7	11	NULL	NULL	NULL	statement 1	Process		prevents					polyadenylation	Process	specific			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_6_2026_s_328	11238938	(B) Binding of fip1-206 to Pap1 prevents specific polyadenylation.	bind
81042	1	3643	11	NULL	NULL	0	NULL	fip1-206	Protein		binds to 					Pap1 	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_6_2026_s_328	11238938	(B) Binding of fip1-206 to Pap1 prevents specific polyadenylation.	bind
81043	2	3643	11	NULL	NULL	0	NULL	statement 1	Process		prevents					polyadenylation	Process	specific			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_6_2026_s_328	11238938	(B) Binding of fip1-206 to Pap1 prevents specific polyadenylation.	bind
8270	1	3644	6	11	NULL	NULL	NULL	Fli1	GP		bind					collagenase	GP	human		tandem elements	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_7_2467_s_138	16537893	(B) Binding of Fli1 and Fos-Jun to the human collagenase tandem  elements.	bind
8271	2	3644	6	11	NULL	NULL	NULL	Fos-Jun	GP		bind					collagenase	GP	human		tandem elements	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_7_2467_s_138	16537893	(B) Binding of Fli1 and Fos-Jun to the human collagenase tandem  elements.	bind
11952	1	3644	7	11	NULL	NULL	NULL	Fli1	GP		bind					collagenase	GP	human		tandem elements	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_7_2467_s_138	16537893	(B) Binding of Fli1 and Fos-Jun to the human collagenase tandem  elements.	bind
11953	2	3644	7	11	NULL	NULL	NULL	Fos-Jun	GP		bind					collagenase	GP	human		tandem elements	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_7_2467_s_138	16537893	(B) Binding of Fli1 and Fos-Jun to the human collagenase tandem  elements.	bind
81044	1	3644	11	NULL	NULL	0	NULL	Fli1	Protein		binds to 					collagenase tandem element	GeneOrProtein	human			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_7_2467_s_138	16537893	(B) Binding of Fli1 and Fos-Jun to the human collagenase tandem  elements.	bind
81045	2	3644	11	NULL	NULL	0	NULL	Fos-Jun	Protein		binds to 					collagenase tandem element	GeneOrProtein	human			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_7_2467_s_138	16537893	(B) Binding of Fli1 and Fos-Jun to the human collagenase tandem  elements.	bind
8272	1	3645	6	11	NULL	NULL	NULL	GAGA protein	GP		bind					iab-7	GP			PRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_4_1311_s_173	11158316	(B) Binding of GAGA protein to the  iab-7 PRE depends on the two consensus GAGA binding sites.	bind
8273	2	3645	6	11	NULL	NULL	NULL	statement 1	Process		depends on							consensus		GAGA binding sites	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_4_1311_s_173	11158316	(B) Binding of GAGA protein to the  iab-7 PRE depends on the two consensus GAGA binding sites.	bind
11954	1	3645	7	11	NULL	NULL	NULL	GAGA protein	GP		bind					 iab-7	GP			PRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_4_1311_s_173	11158316	(B) Binding of GAGA protein to the  iab-7 PRE depends on the two consensus GAGA binding sites.	bind
11955	2	3645	7	11	NULL	NULL	NULL	statement 1	Process		depends on							consensus		GAGA binding site	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_4_1311_s_173	11158316	(B) Binding of GAGA protein to the  iab-7 PRE depends on the two consensus GAGA binding sites.	bind
81046	1	3645	11	NULL	NULL	0	NULL	GAGA protein	Protein		binds to 					iab-7 PRE 	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1311_s_173	11158316	(B) Binding of GAGA protein to the  iab-7 PRE depends on the two consensus GAGA binding sites.	bind
81047	2	3645	11	NULL	NULL	0	NULL	statement 1	Process		depends on					GAGA binding site		consensus			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1311_s_173	11158316	(B) Binding of GAGA protein to the  iab-7 PRE depends on the two consensus GAGA binding sites.	bind
8274	1	3646	6	11	NULL	NULL	NULL	Gal4-VP16	GP		bind					H2A nucleosomes	GP	conventional			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_3_1156_s_120	16428466	(B) Binding of Gal4-VP16 to conventional H2A nucleosomes.	bind
11956	1	3646	7	11	NULL	NULL	NULL	Gal4-VP16	GP		bind					H2A nucleosomes	GP	conventional			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_3_1156_s_120	16428466	(B) Binding of Gal4-VP16 to conventional H2A nucleosomes.	bind
81048	1	3646	11	NULL	NULL	0	NULL	Gal4-VP16	Protein		binds to 					H2A nucleosomes	CellComponent	conventional			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_3_1156_s_120	16428466	(B) Binding of Gal4-VP16 to conventional H2A nucleosomes.	bind
8275	1	3647	6	11	NULL	NULL	NULL	GAS41	GP		bind					p14 ARF gene	GP			promoter	NULL	unstressed IMR-90 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4006_s_228	16705155	(B) Binding of GAS41 to the  p14 ARF gene promoter in unstressed IMR-90 cells.	bind
11957	1	3647	7	11	NULL	NULL	NULL	GAS41	GP		bind					p14 ARF gene	GP			promoter	NULL	unstressed IMR-90 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4006_s_228	16705155	(B) Binding of GAS41 to the  p14 ARF gene promoter in unstressed IMR-90 cells.	bind
81049	1	3647	11	NULL	NULL	0	NULL	GAS41	Protein		binds to 					p14 ARF gene promoter	NucleicAcidSubstance				NULL	in unstressed IMR-90 cells	0	NULL	NULL	NULL	gw70_molcellbiol_26_11_4006_s_228	16705155	(B) Binding of GAS41 to the  p14 ARF gene promoter in unstressed IMR-90 cells.	bind
81050	1	3648	11	NULL	NULL	0	NULL	GST fusion protein	Protein		binds to 					chitin	Chemical				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_64_2_472_s_171	9464381	(b) Binding of GST fusion protein to chitin, chitosan, and Avicel.	bind
81051	2	3648	11	NULL	NULL	0	NULL	GST fusion protein	Protein		binds to 					chitosan	Chemical				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_64_2_472_s_171	9464381	(b) Binding of GST fusion protein to chitin, chitosan, and Avicel.	bind
81052	3	3648	11	NULL	NULL	0	NULL	GST fusion protein	Protein		binds to 					Avicel	Chemical				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_64_2_472_s_171	9464381	(b) Binding of GST fusion protein to chitin, chitosan, and Avicel.	bind
8279	1	3649	6	11	NULL	NULL	NULL	AR protein	GP	deletion mutant	bind					Hey1	GP	35S-labeled			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_4_1425_s_137	15684393	(B) Binding of GST fusion proteins of AR deletion mutants to  35S-labeled Hey1.	bind
53017	2	3649	6	11	NULL	NULL	NULL	AR protein	GP		is a type of					GST fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_4_1425_s_137	15684393	(B) Binding of GST fusion proteins of AR deletion mutants to  35S-labeled Hey1.	bind
11961	1	3649	7	11	NULL	NULL	NULL	AR protein	GP	deletion mutant	bind					Hey1	GP	35S-labeled			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_4_1425_s_137	15684393	(B) Binding of GST fusion proteins of AR deletion mutants to  35S-labeled Hey1.	bind
53019	2	3649	7	11	NULL	NULL	NULL	AR protein	GP		is a type of					GST fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_4_1425_s_137	15684393	(B) Binding of GST fusion proteins of AR deletion mutants to  35S-labeled Hey1.	bind
81053	1	3649	11	NULL	NULL	0	NULL	GST fusion proteins	Protein	AR deletion mutant	binds to 					Hey1	Protein	 35S-labeled 			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_4_1425_s_137	15684393	(B) Binding of GST fusion proteins of AR deletion mutants to  35S-labeled Hey1.	bind
8304	1	3650	6	11	NULL	NULL	NULL	GST-Rab9	GP		bind					GM130	GP				NULL	rat liver Golgi detergent extracts	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
8758	2	3650	6	11	NULL	NULL	NULL	GST-Rab9	GP		bind					golgin-84	GP				NULL	rat liver Golgi detergent extracts	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
8759	3	3650	6	11	NULL	NULL	NULL	GST-Rab9	GP		bind					p115	GP				NULL	rat liver Golgi detergent extracts	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
8760	4	3650	6	11	NULL	NULL	NULL	GST-Rab1	GP		bind					GM130	GP				NULL	rat liver Golgi detergent extracts	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
8761	5	3650	6	11	NULL	NULL	NULL	GST-Rab1	GP		bind					golgin-84	GP				NULL	rat liver Golgi detergent extracts	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
8762	6	3650	6	11	NULL	NULL	NULL	GST-Rab1	GP		bind					p115	GP				NULL	rat liver Golgi detergent extracts	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
8763	7	3650	6	11	NULL	NULL	NULL	GST-Rab9/1	GP		bind					GM130	GP				NULL	rat liver Golgi detergent extracts	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
8764	8	3650	6	11	NULL	NULL	NULL	GST-Rab9/1	GP		bind					golgin-84	GP				NULL	rat liver Golgi detergent extracts	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
8765	9	3650	6	11	NULL	NULL	NULL	GST-Rab9/1	GP		bind					p115	GP				NULL	rat liver Golgi detergent extracts	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
8766	10	3650	6	11	NULL	NULL	NULL	GST-Rab1/9	GP		bind					GM130	GP				NULL	rat liver Golgi detergent extracts	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
8767	11	3650	6	11	NULL	NULL	NULL	GST-Rab1/9	GP		bind					golgin-84	GP				NULL	rat liver Golgi detergent extracts	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
8768	12	3650	6	11	NULL	NULL	NULL	GST-Rab1/9	GP		bind					p115	GP				NULL	rat liver Golgi detergent extracts	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
53022	13	3650	6	11	NULL	NULL	NULL	GM130	GP		is a type of					Rab1 effector	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
53023	14	3650	6	11	NULL	NULL	NULL	golgin-84	GP		is a type of					Rab1 effector	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
53024	15	3650	6	11	NULL	NULL	NULL	p115	GP		is a type of					Rab1 effector	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
11962	1	3650	7	11	NULL	NULL	NULL	GST-Rab9	GP		bind					GM130	GP				NULL	rat liver Golgi detergent extracts	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
11963	2	3650	7	11	NULL	NULL	NULL	GST-Rab1	GP		bind					GM130	GP				NULL	rat liver Golgi detergent extracts	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
11964	3	3650	7	11	NULL	NULL	NULL	GST-Rab9/1	GP		bind					GM130	GP				NULL	rat liver Golgi detergent extracts	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
11965	4	3650	7	11	NULL	NULL	NULL	GST-Rab1/9	GP		bind					GM130	GP				NULL	rat liver Golgi detergent extracts	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
11966	5	3650	7	11	NULL	NULL	NULL	GST-Rab9	GP		bind					golgin-84	GP				NULL	rat liver Golgi detergent extracts	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
11967	6	3650	7	11	NULL	NULL	NULL	GST-Rab1	GP		bind					golgin-84	GP				NULL	rat liver Golgi detergent extracts	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
11968	7	3650	7	11	NULL	NULL	NULL	GST-Rab9/1	GP		bind					golgin-84	GP				NULL	rat liver Golgi detergent extracts	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
11969	8	3650	7	11	NULL	NULL	NULL	GST-Rab1/9	GP		bind					golgin-84	GP				NULL	rat liver Golgi detergent extracts	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
11970	9	3650	7	11	NULL	NULL	NULL	GST-Rab9	GP		bind					p115	GP				NULL	rat liver Golgi detergent extracts	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
11971	10	3650	7	11	NULL	NULL	NULL	GST-Rab1	GP		bind					 p115 	GP				NULL	rat liver Golgi detergent extracts	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
11972	11	3650	7	11	NULL	NULL	NULL	GST-Rab9/1	GP		bind					p115	GP				NULL	rat liver Golgi detergent extracts	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
11973	12	3650	7	11	NULL	NULL	NULL	GST-Rab1/9	GP		bind					p115	GP				NULL	rat liver Golgi detergent extracts	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
11974	13	3650	7	11	NULL	NULL	NULL	GM130	GP		is a type of					Rab1 effector	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
11975	14	3650	7	11	NULL	NULL	NULL	golgin-84	GP		is a type of					Rab1 effector	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
11976	15	3650	7	11	NULL	NULL	NULL	p115	GP		is a type of					Rab1 effector	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
81054	1	3650	11	NULL	NULL	0	NULL	Rab1	Protein		binds to 					GM130	Protein	Golgi detergent extract			NULL	rat liver	0	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
81055	2	3650	11	NULL	NULL	0	NULL	Rab1	Protein		binds to 					golgin-84	Protein	Golgi detergent extract			NULL	rat liver	0	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
81056	3	3650	11	NULL	NULL	0	NULL	Rab1	Protein		binds to 					p115	Protein	Golgi detergent extract			NULL	rat liver	0	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
81057	4	3650	11	NULL	NULL	0	NULL	Rab9	Protein	GST version	binds to 					GM130	Protein	Golgi detergent extract			NULL	rat liver	0	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
81058	5	3650	11	NULL	NULL	0	NULL	 Rab9	Protein	GST version	binds to 					golgin-84	Protein	Golgi detergent extract			NULL	rat liver	0	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
81059	6	3650	11	NULL	NULL	0	NULL	 Rab9	Protein	GST version	binds to 					p115	Protein	Golgi detergent extract			NULL	rat liver	0	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
81060	7	3650	11	NULL	NULL	0	NULL	Rab1	Protein	GST version	binds to 					GM130	Protein	Golgi detergent extract			NULL	rat liver	0	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
81061	8	3650	11	NULL	NULL	0	NULL	Rab1	Protein	GST version	binds to 					golgin-84	Protein	Golgi detergent extract			NULL	rat liver	0	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
81062	9	3650	11	NULL	NULL	0	NULL	Rab1	Protein	GST version	binds to 					p115	Protein	Golgi detergent extract			NULL	rat liver	0	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
81063	10	3650	11	NULL	NULL	0	NULL	Rab9/1	Protein	GST version	binds to 					GM130	Protein	Golgi detergent extract			NULL	rat liver	0	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
81064	11	3650	11	NULL	NULL	NULL	NULL	Rab9/1	Protein	GST version	binds to 					p115	Protein	Golgi detergent extract			NULL	rat liver	NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
81065	12	3650	11	NULL	NULL	0	NULL	Rab9/1	Protein	GST version	binds to 					golgin-84	Protein	Golgi detergent extract			NULL	rat liver	0	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
81066	13	3650	11	NULL	NULL	0	NULL	Rab1/9	Protein	GST version	binds to 					GM130	Protein	Golgi detergent extract			NULL	rat liver	0	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
81067	14	3650	11	NULL	NULL	0	NULL	Rab1/9	Protein	GST version	binds to 					golgin-84	Protein	Golgi detergent extract			NULL	rat liver	0	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
81068	15	3650	11	NULL	NULL	0	NULL	Rab1/9	Protein	GST version	binds to 					p115	Protein	Golgi detergent extract			NULL	rat liver	0	NULL	NULL	NULL	gw70_cellbiol_173_6_917_s_78	16769818	(B) Binding of GST versions of Rab9, Rab1, Rab9/1, and  Rab1/9 to Rab1 effectors GM130, golgin-84, and p115 from rat liver Golgi detergent  extracts.	bind
8305	1	3651	6	11	NULL	NULL	NULL	Cdc42	GP	GTP-loaded 	bind					PAK1	GP		PBD		NULL		NULL	NULL	NULL	NULL	gw60_cell_102_3_387_s_242	10975528	(B) Binding of GTP-loaded Cdc42 (or Rac) with the PAK1 p21 binding domain  (PBD) disrupts the dimer and unfolds the IS domain (symbolized by its reversion  to a formless oval).	bind
8306	2	3651	6	11	NULL	NULL	NULL	Rac	GP	GTP-loaded	bind					PAK1	GP		PBD		NULL		NULL	NULL	NULL	NULL	gw60_cell_102_3_387_s_242	10975528	(B) Binding of GTP-loaded Cdc42 (or Rac) with the PAK1 p21 binding domain  (PBD) disrupts the dimer and unfolds the IS domain (symbolized by its reversion  to a formless oval).	bind
8307	3	3651	6	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_102_3_387_s_242	10975528	(B) Binding of GTP-loaded Cdc42 (or Rac) with the PAK1 p21 binding domain  (PBD) disrupts the dimer and unfolds the IS domain (symbolized by its reversion  to a formless oval).	bind
8308	4	3651	6	11	NULL	NULL	NULL	PBD	GP		is					p21 binding domain	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_102_3_387_s_242	10975528	(B) Binding of GTP-loaded Cdc42 (or Rac) with the PAK1 p21 binding domain  (PBD) disrupts the dimer and unfolds the IS domain (symbolized by its reversion  to a formless oval).	bind
8309	5	3651	6	11	NULL	NULL	NULL	statement 1	Process		disrupts					dimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_102_3_387_s_242	10975528	(B) Binding of GTP-loaded Cdc42 (or Rac) with the PAK1 p21 binding domain  (PBD) disrupts the dimer and unfolds the IS domain (symbolized by its reversion  to a formless oval).	bind
8310	6	3651	6	11	NULL	NULL	NULL	statement 2	Process		disrupts					dimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_102_3_387_s_242	10975528	(B) Binding of GTP-loaded Cdc42 (or Rac) with the PAK1 p21 binding domain  (PBD) disrupts the dimer and unfolds the IS domain (symbolized by its reversion  to a formless oval).	bind
8311	7	3651	6	11	NULL	NULL	NULL	statement 1	Process		unfolds								IS domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_102_3_387_s_242	10975528	(B) Binding of GTP-loaded Cdc42 (or Rac) with the PAK1 p21 binding domain  (PBD) disrupts the dimer and unfolds the IS domain (symbolized by its reversion  to a formless oval).	bind
8312	8	3651	6	11	NULL	NULL	NULL	statement 2	Process		unfolds								IS domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_102_3_387_s_242	10975528	(B) Binding of GTP-loaded Cdc42 (or Rac) with the PAK1 p21 binding domain  (PBD) disrupts the dimer and unfolds the IS domain (symbolized by its reversion  to a formless oval).	bind
11977	1	3651	7	11	NULL	NULL	NULL	Cdc42	GP	GTP-loaded	bind					PAK1	GP		p21 binding domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_102_3_387_s_242	10975528	(B) Binding of GTP-loaded Cdc42 (or Rac) with the PAK1 p21 binding domain  (PBD) disrupts the dimer and unfolds the IS domain (symbolized by its reversion  to a formless oval).	bind
11978	2	3651	7	11	NULL	NULL	NULL	Rac	GP	GTP-loaded	bind					PAK1	GP		p21 binding domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_102_3_387_s_242	10975528	(B) Binding of GTP-loaded Cdc42 (or Rac) with the PAK1 p21 binding domain  (PBD) disrupts the dimer and unfolds the IS domain (symbolized by its reversion  to a formless oval).	bind
11979	3	3651	7	11	NULL	NULL	NULL	statement 1	Process		disrupts					dimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_102_3_387_s_242	10975528	(B) Binding of GTP-loaded Cdc42 (or Rac) with the PAK1 p21 binding domain  (PBD) disrupts the dimer and unfolds the IS domain (symbolized by its reversion  to a formless oval).	bind
11980	4	3651	7	11	NULL	NULL	NULL	statement 1	Process		unfolds								IS domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_102_3_387_s_242	10975528	(B) Binding of GTP-loaded Cdc42 (or Rac) with the PAK1 p21 binding domain  (PBD) disrupts the dimer and unfolds the IS domain (symbolized by its reversion  to a formless oval).	bind
11981	5	3651	7	11	NULL	NULL	NULL	statement 2	Process		disrupts					dimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_102_3_387_s_242	10975528	(B) Binding of GTP-loaded Cdc42 (or Rac) with the PAK1 p21 binding domain  (PBD) disrupts the dimer and unfolds the IS domain (symbolized by its reversion  to a formless oval).	bind
11982	6	3651	7	11	NULL	NULL	NULL	statement 2	Process		unfolds								IS domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_102_3_387_s_242	10975528	(B) Binding of GTP-loaded Cdc42 (or Rac) with the PAK1 p21 binding domain  (PBD) disrupts the dimer and unfolds the IS domain (symbolized by its reversion  to a formless oval).	bind
11983	7	3651	7	11	NULL	NULL	NULL	p21 binding domain	GP		is					PBD	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_102_3_387_s_242	10975528	(B) Binding of GTP-loaded Cdc42 (or Rac) with the PAK1 p21 binding domain  (PBD) disrupts the dimer and unfolds the IS domain (symbolized by its reversion  to a formless oval).	bind
53026	8	3651	7	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_102_3_387_s_242	10975528	(B) Binding of GTP-loaded Cdc42 (or Rac) with the PAK1 p21 binding domain  (PBD) disrupts the dimer and unfolds the IS domain (symbolized by its reversion  to a formless oval).	bind
81069	1	3651	11	NULL	NULL	0	NULL	Cdc42	Protein	GTP-loaded	binds to 					PAK1	Protein		p21 binding domain		NULL		0	NULL	NULL	NULL	gw60_cell_102_3_387_s_242	10975528	(B) Binding of GTP-loaded Cdc42 (or Rac) with the PAK1 p21 binding domain  (PBD) disrupts the dimer and unfolds the IS domain (symbolized by its reversion  to a formless oval).	bind
81070	2	3651	11	NULL	NULL	0	NULL	p21 binding domain	PartOfProtein		is					PBD	PartOfProtein				NULL		0	NULL	NULL	NULL	gw60_cell_102_3_387_s_242	10975528	(B) Binding of GTP-loaded Cdc42 (or Rac) with the PAK1 p21 binding domain  (PBD) disrupts the dimer and unfolds the IS domain (symbolized by its reversion  to a formless oval).	bind
81071	3	3651	11	NULL	NULL	0	NULL	Rac	Protein		binds to 					 PAK1	Protein		p21 binding domain		NULL		0	NULL	NULL	NULL	gw60_cell_102_3_387_s_242	10975528	(B) Binding of GTP-loaded Cdc42 (or Rac) with the PAK1 p21 binding domain  (PBD) disrupts the dimer and unfolds the IS domain (symbolized by its reversion  to a formless oval).	bind
8317	1	3652	6	11	NULL	NULL	NULL	H6-CodY	GP		bind					P oppD fragment	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_187_2_512_s_202	15629923	(B) Binding of H6-CodY to labeled PCR products encompassing the mutated promoter  regions presented in panel A in an in vitro binding assay, relative to its binding  to the wild-type P oppD fragment.	bind
11985	1	3652	7	11	NULL	NULL	NULL	H6-CodY	GP		bind					P oppD fragment	GP	wild-type			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_187_2_512_s_202	15629923	(B) Binding of H6-CodY to labeled PCR products encompassing the mutated promoter  regions presented in panel A in an in vitro binding assay, relative to its binding  to the wild-type P oppD fragment.	bind
81072	1	3652	11	NULL	NULL	0	NULL	H6-CodY	Protein		binds to 					labeled PCR product	SmallMolecule				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_2_512_s_202	15629923	(B) Binding of H6-CodY to labeled PCR products encompassing the mutated promoter  regions presented in panel A in an in vitro binding assay, relative to its binding  to the wild-type P oppD fragment.	bind
8321	1	3653	6	11	NULL	NULL	NULL	Hsp40	GP		bind					GST-70C139	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2023_s_142	9528774	(B) Binding of Hsp40 to GST-70C139 was performed in the absence ( ) of Hsc70 or in the presence (+) of equimolar amounts of Hsc70 and the GST fusion protein, and Hsp40 was detected in the flowthrough fractions by Coomassie blue staining.	bind
11986	1	3653	7	11	NULL	NULL	NULL	Hsp40	GP		bind					GST-70C139	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2023_s_142	9528774	(B) Binding of Hsp40 to GST-70C139 was performed in the absence ( ) of Hsc70 or in the presence (+) of equimolar amounts of Hsc70 and the GST fusion protein, and Hsp40 was detected in the flowthrough fractions by Coomassie blue staining.	bind
81073	1	3653	11	NULL	NULL	0	NULL	Hsp40	Protein		binds to 					GST-70C139	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_4_2023_s_142	9528774	(B) Binding of Hsp40 to GST-70C139 was performed in the absence ( ) of Hsc70 or in the presence (+) of equimolar amounts of Hsc70 and the GST fusion protein, and Hsp40 was detected in the flowthrough fractions by Coomassie blue staining.	bind
81075	2	3653	11	NULL	NULL	NULL	NULL	Hsp40	Protein		was detected in					Coomassie blue staining	ResearchActivity	flowthrough fraction by			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2023_s_142	9528774	(B) Binding of Hsp40 to GST-70C139 was performed in the absence ( ) of Hsc70 or in the presence (+) of equimolar amounts of Hsc70 and the GST fusion protein, and Hsp40 was detected in the flowthrough fractions by Coomassie blue staining.	bind
8322	1	3654	6	11	NULL	NULL	NULL	IgG fractions	GP		bind					RO	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_1_11_s_105	9423833	(B) Binding of IgG fractions to R0; (C) binding of IgG fractions to R2-coated plates.	bind
8324	2	3654	6	11	NULL	NULL	NULL	IgG fractions	GP		bind					R2	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_1_11_s_105	9423833	(B) Binding of IgG fractions to R0; (C) binding of IgG fractions to R2-coated plates.	bind
11987	1	3654	7	11	NULL	NULL	NULL	IgG fractions	GP		bind					R0	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_1_11_s_105	9423833	(B) Binding of IgG fractions to R0; (C) binding of IgG fractions to R2-coated plates.	bind
11988	2	3654	7	11	NULL	NULL	NULL	IgG fraction	GP		bind					R2	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_1_11_s_105	9423833	(B) Binding of IgG fractions to R0; (C) binding of IgG fractions to R2-coated plates.	bind
81076	1	3654	11	NULL	NULL	0	NULL	IgG fraction	PartOfProtein		binds to 					R0	PartOfProtein				NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_1_11_s_105	9423833	(B) Binding of IgG fractions to R0; (C) binding of IgG fractions to R2-coated plates.	bind
81077	2	3654	11	NULL	NULL	0	NULL	IgG fraction	PartOfProtein		binds to 					R2	PartOfProtein				NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_1_11_s_105	9423833	(B) Binding of IgG fractions to R0; (C) binding of IgG fractions to R2-coated plates.	bind
8326	1	3656	6	11	NULL	NULL	NULL	IRF-3	GP		bind					importin-alpha receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_11_4159_s_234	10805757	(B) Binding of IRF-3 to importin-alpha receptors is NLS specific.	bind
11989	1	3656	7	NULL	NULL	0	NULL	IRF-3	NULL		bind	NULL				importin-alpha receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_11_4159_s_234	10805757	(B) Binding of IRF-3 to importin-alpha receptors is NLS specific.	bind
11990	2	3656	7	NULL	NULL	0	NULL	statement 1	NULL		is specific to	NULL				NLS	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_11_4159_s_234	10805757	(B) Binding of IRF-3 to importin-alpha receptors is NLS specific.	bind
81078	1	3656	11	NULL	NULL	0	NULL	IRF-3	Protein		binds to 					importin-alpha receptor	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_11_4159_s_234	10805757	(B) Binding of IRF-3 to importin-alpha receptors is NLS specific.	bind
81079	2	3656	11	NULL	NULL	0	NULL	statement 1	Process		is specific to					NLS	AminoAcid				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_11_4159_s_234	10805757	(B) Binding of IRF-3 to importin-alpha receptors is NLS specific.	bind
8327	2	3657	6	11	NULL	NULL	NULL	statement 1	Process		is specific to					NLS	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_87_5_881_s_126	8945515	(B) Binding of labeled E. coli DnaB to  the GST, GST - wtRTP, and GST - mutant RTP matrices.	bind
8329	1	3657	6	11	NULL	NULL	NULL	DnaB	GP	labeled;; E. coli	bind					GST	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_87_5_881_s_126	8945515	(B) Binding of labeled E. coli DnaB to  the GST, GST - wtRTP, and GST - mutant RTP matrices.	bind
8330	2	3657	6	11	NULL	NULL	NULL	DnaB	GP	labeled;; E. coli	bind					GST-RTP	GP	wt			NULL		NULL	NULL	NULL	NULL	gw60_cell_87_5_881_s_126	8945515	(B) Binding of labeled E. coli DnaB to  the GST, GST - wtRTP, and GST - mutant RTP matrices.	bind
8331	3	3657	6	11	NULL	NULL	NULL	DnaB	GP	labeled;; E. coli	bind					GST-RTP	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_cell_87_5_881_s_126	8945515	(B) Binding of labeled E. coli DnaB to  the GST, GST - wtRTP, and GST - mutant RTP matrices.	bind
11992	2	3657	7	11	NULL	NULL	NULL	DnaB	GP	labeled;; E. coli	bind					GST - RTP	GP	wt			NULL		NULL	NULL	NULL	NULL	gw60_cell_87_5_881_s_126	8945515	(B) Binding of labeled E. coli DnaB to  the GST, GST - wtRTP, and GST - mutant RTP matrices.	bind
11993	3	3657	7	11	NULL	NULL	NULL	DnaB	GP	labeled;; E. coli	bind					GST - RTP	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_cell_87_5_881_s_126	8945515	(B) Binding of labeled E. coli DnaB to  the GST, GST - wtRTP, and GST - mutant RTP matrices.	bind
81080	1	3657	11	NULL	NULL	0	NULL	DnaB	Protein	labeled E. coli	binds to 					GST	Protein				NULL		0	NULL	NULL	NULL	gw60_cell_87_5_881_s_126	8945515	(B) Binding of labeled E. coli DnaB to  the GST, GST - wtRTP, and GST - mutant RTP matrices.	bind
81081	2	3657	11	NULL	NULL	0	NULL	 DnaB	Protein	labeled E. coli	binds to 					GST - wtRTP	Protein				NULL		0	NULL	NULL	NULL	gw60_cell_87_5_881_s_126	8945515	(B) Binding of labeled E. coli DnaB to  the GST, GST - wtRTP, and GST - mutant RTP matrices.	bind
81082	3	3657	11	NULL	NULL	0	NULL	DnaB	Protein	labeled E. coli	binds to 					GST - mutant RTP	Protein				NULL		0	NULL	NULL	NULL	gw60_cell_87_5_881_s_126	8945515	(B) Binding of labeled E. coli DnaB to  the GST, GST - wtRTP, and GST - mutant RTP matrices.	bind
8334	1	3658	6	11	NULL	NULL	NULL	LIS1	GP		bind					GST-mNudE	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_28_3_665_s_90	11163258	(B) Binding of LIS1 to GST-mNudE.	bind
11994	1	3658	7	11	NULL	NULL	NULL	LIS1	GP		bind					GST-mNudE	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_28_3_665_s_90	11163258	(B) Binding of LIS1 to GST-mNudE.	bind
81083	1	3658	11	NULL	NULL	0	NULL	LIS1	Protein		binds to 					GST-mNudE	Protein				NULL		0	NULL	NULL	NULL	gw60_neuron_28_3_665_s_90	11163258	(B) Binding of LIS1 to GST-mNudE.	bind
8339	1	3659	6	11	NULL	NULL	NULL	 MdcR	GP		bind					P mdcR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_7_2302_s_87	10094715	(B) Binding of MdcR to P mdcR.	bind
11991	1	3659	7	11	NULL	NULL	NULL	DnaB	GP	labeled;; E. coli	bind					GST	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_7_2302_s_87	10094715	(B) Binding of MdcR to P mdcR.	bind
11995	1	3659	7	11	NULL	NULL	NULL	MdcR	GP		bind					P mdcR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_7_2302_s_87	10094715	(B) Binding of MdcR to P mdcR.	bind
81084	1	3659	11	NULL	NULL	0	NULL	MdcR	Gene		binds to 					P mdcR	Protein				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_7_2302_s_87	10094715	(B) Binding of MdcR to P mdcR.	bind
8342	1	3660	6	11	NULL	NULL	NULL	MDMX 	GP		bind					MDM2	GP	point mutants			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_15_5113_s_126	12860999	(B) Binding of MDMX to MDM2 point mutants.	bind
11996	1	3660	7	11	NULL	NULL	NULL	MDMX	GP		bind					MDM2	GP	point mutant			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_15_5113_s_126	12860999	(B) Binding of MDMX to MDM2 point mutants.	bind
81085	1	3660	11	NULL	NULL	0	NULL	MDMX	Protein		binds to 					MDM2 point mutant	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_15_5113_s_126	12860999	(B) Binding of MDMX to MDM2 point mutants.	bind
8344	1	3661	6	11	NULL	NULL	NULL	MEF2D	GP	in vitro-translated;;35S-labeled	bind					HDAC7	GP		C-ter		NULL		NULL	NULL	NULL	NULL	gw60_immunity_18_5_687_s_134	12753745	(B) Binding of MEF2D to the carboxyl (C-ter) or amino (N-ter) terminus of HDAC7 was measured in pull-down assays with in vitro translated 35S-labeled MEF2D.	bind
8345	2	3661	6	11	NULL	NULL	NULL	MEF2D	GP	in vitro-translated;;35S-labeled	bind					HDAC7	GP		N-ter		NULL		NULL	NULL	NULL	NULL	gw60_immunity_18_5_687_s_134	12753745	(B) Binding of MEF2D to the carboxyl (C-ter) or amino (N-ter) terminus of HDAC7 was measured in pull-down assays with in vitro translated 35S-labeled MEF2D.	bind
8346	3	3661	6	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_18_5_687_s_134	12753745	(B) Binding of MEF2D to the carboxyl (C-ter) or amino (N-ter) terminus of HDAC7 was measured in pull-down assays with in vitro translated 35S-labeled MEF2D.	bind
40911	4	3661	6	11	NULL	NULL	NULL	C-ter	AminoAcid		is					Carboxyl terminus	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_immunity_18_5_687_s_134	12753745	(B) Binding of MEF2D to the carboxyl (C-ter) or amino (N-ter) terminus of HDAC7 was measured in pull-down assays with in vitro translated 35S-labeled MEF2D.	bind
40912	5	3661	6	11	NULL	NULL	NULL	N-ter	AminoAcid		is					amino terminus	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_immunity_18_5_687_s_134	12753745	(B) Binding of MEF2D to the carboxyl (C-ter) or amino (N-ter) terminus of HDAC7 was measured in pull-down assays with in vitro translated 35S-labeled MEF2D.	bind
12076	1	3661	7	11	NULL	NULL	NULL	 MEF2D	GP	in vitro translated;;35S-labeled	bind					HDAC7	GP		 amino terminus		NULL		NULL	NULL	NULL	NULL	gw60_immunity_18_5_687_s_134	12753745	(B) Binding of MEF2D to the carboxyl (C-ter) or amino (N-ter) terminus of HDAC7 was measured in pull-down assays with in vitro translated 35S-labeled MEF2D.	bind
12077	2	3661	7	11	NULL	NULL	NULL	MEF2D	GP	in vitro-translated;;35S labeled	bind					HDAC7	GP		carboxyl terminus		NULL		NULL	NULL	NULL	NULL	gw60_immunity_18_5_687_s_134	12753745	(B) Binding of MEF2D to the carboxyl (C-ter) or amino (N-ter) terminus of HDAC7 was measured in pull-down assays with in vitro translated 35S-labeled MEF2D.	bind
12078	3	3661	7	11	NULL	NULL	NULL	carboxyl terminus	AminoAcid		is					C-ter	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_immunity_18_5_687_s_134	12753745	(B) Binding of MEF2D to the carboxyl (C-ter) or amino (N-ter) terminus of HDAC7 was measured in pull-down assays with in vitro translated 35S-labeled MEF2D.	bind
12079	4	3661	7	11	NULL	NULL	NULL	amino terminus	AminoAcid		is					N-ter	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_immunity_18_5_687_s_134	12753745	(B) Binding of MEF2D to the carboxyl (C-ter) or amino (N-ter) terminus of HDAC7 was measured in pull-down assays with in vitro translated 35S-labeled MEF2D.	bind
15050	5	3661	7	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_18_5_687_s_134	12753745	(B) Binding of MEF2D to the carboxyl (C-ter) or amino (N-ter) terminus of HDAC7 was measured in pull-down assays with in vitro translated 35S-labeled MEF2D.	bind
81086	1	3661	11	NULL	NULL	0	NULL	MEF2D	Protein		binds to 					HDAC7	Protein		carboxyl terminus		NULL		0	NULL	NULL	NULL	gw60_immunity_18_5_687_s_134	12753745	(B) Binding of MEF2D to the carboxyl (C-ter) or amino (N-ter) terminus of HDAC7 was measured in pull-down assays with in vitro translated 35S-labeled MEF2D.	bind
81087	2	3661	11	NULL	NULL	0	NULL	MEF2D	Protein		binds to 					HDAC7	Protein		amino terminus		NULL		0	NULL	NULL	NULL	gw60_immunity_18_5_687_s_134	12753745	(B) Binding of MEF2D to the carboxyl (C-ter) or amino (N-ter) terminus of HDAC7 was measured in pull-down assays with in vitro translated 35S-labeled MEF2D.	bind
81088	3	3661	11	NULL	NULL	0	NULL	statement 1	Process		was measured in					pull-down assay	LaboratoryExperimentalFactor				NULL		0	NULL	NULL	NULL	gw60_immunity_18_5_687_s_134	12753745	(B) Binding of MEF2D to the carboxyl (C-ter) or amino (N-ter) terminus of HDAC7 was measured in pull-down assays with in vitro translated 35S-labeled MEF2D.	bind
81089	4	3661	11	NULL	NULL	0	NULL	statement 2	Process		measured in					pull-down assay	LaboratoryExperimentalFactor				NULL		0	NULL	NULL	NULL	gw60_immunity_18_5_687_s_134	12753745	(B) Binding of MEF2D to the carboxyl (C-ter) or amino (N-ter) terminus of HDAC7 was measured in pull-down assays with in vitro translated 35S-labeled MEF2D.	bind
8347	1	3662	6	11	NULL	NULL	NULL	MKL1	GP		bind					SRF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6597_s_128	12944485	(B) Binding of MKL1 to SRF in gel mobility shift assays.	bind
12080	1	3662	7	11	NULL	NULL	NULL	MKL1	GP		bind					SRF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6597_s_128	12944485	(B) Binding of MKL1 to SRF in gel mobility shift assays.	bind
81090	1	3662	11	NULL	NULL	0	NULL	MKL1	Protein		binds to 					SRF	Protein				NULL	gel mobility shift assay	0	NULL	NULL	NULL	gw60_molcellbiol_23_18_6597_s_128	12944485	(B) Binding of MKL1 to SRF in gel mobility shift assays.	bind
8348	1	3663	6	11	NULL	NULL	NULL	MOG-6	GP		bind					MEP-1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_development_131_12_2935_s_129	15151984	(B) Binding of MOG-6 to MEP-1 in vitro.	bind
12081	1	3663	7	11	NULL	NULL	NULL	MOG-6	GP		bind					MEP-1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_development_131_12_2935_s_129	15151984	(B) Binding of MOG-6 to MEP-1 in vitro.	bind
81091	1	3663	11	NULL	NULL	0	NULL	MOG-6	Protein		binds to 					MEP-1	Protein				NULL	in vitro	0	NULL	NULL	NULL	gw70_development_131_12_2935_s_129	15151984	(B) Binding of MOG-6 to MEP-1 in vitro.	bind
8349	1	3664	6	11	NULL	NULL	NULL	n-sec1	GP		bind					syntaxin 1a	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_16_6_1229_s_89	8663999	(B) Binding of n-sec1 to syntaxin 1a in the presence of 500  M S-NC.	bind
8350	2	3664	6	11	NULL	NULL	NULL	statement 1	Process		occurs in presence of					S-NC	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_neuron_16_6_1229_s_89	8663999	(B) Binding of n-sec1 to syntaxin 1a in the presence of 500  M S-NC.	bind
12082	1	3664	7	11	NULL	NULL	NULL	n-sec1	GP		bind					syntaxin 1a	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_16_6_1229_s_89	8663999	(B) Binding of n-sec1 to syntaxin 1a in the presence of 500  M S-NC.	bind
81092	1	3664	11	NULL	NULL	0	NULL	n-sec1	Protein		binds to 					syntaxin 1a	Protein				NULL		0	NULL	NULL	NULL	gw60_neuron_16_6_1229_s_89	8663999	(B) Binding of n-sec1 to syntaxin 1a in the presence of 500  M S-NC.	bind
81093	2	3664	11	NULL	NULL	0	NULL	statement 1	Process		occurs in the presence of					S-nitrosocysteine	AminoAcid				NULL		0	NULL	NULL	NULL	gw60_neuron_16_6_1229_s_89	8663999	(B) Binding of n-sec1 to syntaxin 1a in the presence of 500  M S-NC.	bind
8351	1	3665	6	11	NULL	NULL	NULL	NIF-1	GP		bind					NRC	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_19_6883_s_68	12215545	(B) Binding of NIF-1 with NRC in vitro.	bind
12083	1	3665	7	11	NULL	NULL	NULL	NIF-1	GP		bind					NRC	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_19_6883_s_68	12215545	(B) Binding of NIF-1 with NRC in vitro.	bind
81094	1	3665	11	NULL	NULL	NULL	NULL	NIF-1	Protein		binds to 					NRC	Protein				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_19_6883_s_68	12215545	(B) Binding of NIF-1 with NRC in vitro.	bind
8352	1	3666	6	11	NULL	NULL	NULL	nuclear proteins	GP		bind					Sp1 sites	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1574_2_164_s_207	11955626	(B) Binding of nuclear proteins to both Sp1 sites.	bind
12085	1	3666	7	11	NULL	NULL	NULL	nuclear proteins	GP		bind					Sp1 sites	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1574_2_164_s_207	11955626	(B) Binding of nuclear proteins to both Sp1 sites.	bind
81095	1	3666	11	NULL	NULL	0	NULL	nuclear protein	Protein		binds to 					Sp1 site	Protein				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1574_2_164_s_207	11955626	(B) Binding of nuclear proteins to both Sp1 sites.	bind
8353	1	3667	6	11	NULL	NULL	NULL	nuclear proteins	GP		bind							radiolabeled		B-CRE	NULL		NULL	NULL	NULL	NULL	gw60_neuron_20_4_709_s_254	9581763	(B) Binding of nuclear proteins to radiolabeled B-CRE in an electrophoretic mobility shift assay.	bind
12087	1	3667	7	11	NULL	NULL	NULL	nuclear proteins	GP		bind							 radiolabeled		B-CRE	NULL		NULL	NULL	NULL	NULL	gw60_neuron_20_4_709_s_254	9581763	(B) Binding of nuclear proteins to radiolabeled B-CRE in an electrophoretic mobility shift assay.	bind
81096	1	3667	11	NULL	NULL	0	NULL	nuclear protein	Protein		binds to 					B-CRE	NucleicAcidSubstance	radiolabeled			NULL	electrophoretic mobility shift assay	0	NULL	NULL	NULL	gw60_neuron_20_4_709_s_254	9581763	(B) Binding of nuclear proteins to radiolabeled B-CRE in an electrophoretic mobility shift assay.	bind
8354	1	3668	6	11	NULL	NULL	NULL	p115	GP		bind					CSW	GP		SH2 domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_85_6_899_s_88	8681384	(B) Binding of p115 to the  CSW SH2 domains.	bind
12089	1	3668	7	11	NULL	NULL	NULL	p115	GP		bind					CSW	GP		SH2 domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_85_6_899_s_88	8681384	(B) Binding of p115 to the  CSW SH2 domains.	bind
81097	1	3668	11	NULL	NULL	0	NULL	p115	Protein		binds to 					CSW	Protein		SH2 domain		NULL		0	NULL	NULL	NULL	gw60_cell_85_6_899_s_88	8681384	(B) Binding of p115 to the  CSW SH2 domains.	bind
8355	1	3669	6	11	NULL	NULL	NULL	Pbx1	GP		bind					Hox11	GP			PX1 oligo within the promoter	NULL		NULL	NULL	NULL	NULL	gw70_development_132_13_3113_s_192	15944191	(B) Binding of Pbx1 and Hox11 to the (PX1) oligo within the  Hox11 promoter.	bind
17775	2	3669	6	11	NULL	NULL	NULL	Hox11	GP		bind					Hox11	GP			PX1 oligo within the promoter	NULL		NULL	NULL	NULL	NULL	gw70_development_132_13_3113_s_192	15944191	(B) Binding of Pbx1 and Hox11 to the (PX1) oligo within the  Hox11 promoter.	bind
12091	1	3669	7	11	NULL	NULL	NULL	Pbx1	GP		bind					Hox11	GP			PX1 oligo in the promoter of 	NULL		NULL	NULL	NULL	NULL	gw70_development_132_13_3113_s_192	15944191	(B) Binding of Pbx1 and Hox11 to the (PX1) oligo within the  Hox11 promoter.	bind
12092	2	3669	7	11	NULL	NULL	NULL	Hox11	GP		bind					Hox11	GP			PX1 oligo in the promoter of 	NULL		NULL	NULL	NULL	NULL	gw70_development_132_13_3113_s_192	15944191	(B) Binding of Pbx1 and Hox11 to the (PX1) oligo within the  Hox11 promoter.	bind
81098	1	3669	11	NULL	NULL	0	NULL	Pbx1	Protein		binds to 					Hox11 promoter	NucleicAcidSubstance			PX1 oligo	NULL		0	NULL	NULL	NULL	gw70_development_132_13_3113_s_192	15944191	(B) Binding of Pbx1 and Hox11 to the (PX1) oligo within the  Hox11 promoter.	bind
81099	2	3669	11	NULL	NULL	0	NULL	Hox11	Protein		binds to 					Hox11 promoter	NucleicAcidSubstance			PX1 oligo	NULL		0	NULL	NULL	NULL	gw70_development_132_13_3113_s_192	15944191	(B) Binding of Pbx1 and Hox11 to the (PX1) oligo within the  Hox11 promoter.	bind
8356	1	3670	6	11	NULL	NULL	NULL	Pex7p	GP		bind					PTS2 protein	GP	synthetic			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6056_s_96	12167700	(B) Binding of Pex7p to a synthetic PTS2 protein in vitro.	bind
12093	1	3670	7	11	NULL	NULL	NULL	Pex7p	GP		bind					PTS2 protein	GP	synthetic			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6056_s_96	12167700	(B) Binding of Pex7p to a synthetic PTS2 protein in vitro.	bind
81100	1	3670	11	NULL	NULL	0	NULL	Pex7p	Protein		binds to 					synthetic PTS2 protein	Protein				NULL	in vitro	0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6056_s_96	12167700	(B) Binding of Pex7p to a synthetic PTS2 protein in vitro.	bind
8357	1	3671	6	11	NULL	NULL	NULL	Pex7p	GP		bind					Pex13p	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6056_s_229	12167700	(B) Binding of Pex7p to Pex13p in vitro.	bind
12094	1	3671	7	11	NULL	NULL	NULL	Pex7p	GP		bind					Pex13p	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6056_s_229	12167700	(B) Binding of Pex7p to Pex13p in vitro.	bind
81101	1	3671	11	NULL	NULL	0	NULL	Pex7p	Protein		binds to 					Pex13p	Protein				NULL	in vitro	0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6056_s_229	12167700	(B) Binding of Pex7p to Pex13p in vitro.	bind
81102	1	3672	11	NULL	NULL	0	NULL	protein	Protein		binds to 					consensus AP-1	Protein				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1524_1_57_s_137	11078959	(B) Binding of protein(s) to a consensus AP-1 element was inhibited by exposure of EC to quinacrine.	bind
81103	2	3672	11	NULL	NULL	0	NULL	quinacrine	Chemical	exposure of	inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1524_1_57_s_137	11078959	(B) Binding of protein(s) to a consensus AP-1 element was inhibited by exposure of EC to quinacrine.	bind
12095	1	3673	7	11	NULL	NULL	NULL	Eve protein	GP	purified	bind					GST-dTBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_1_77_s_93	10024881	(b) Binding of purified Eve proteins to GST-dTBP.	bind
81104	1	3673	11	NULL	NULL	0	NULL	Eve protein	Protein	purified	binds to 					GST-dTBP	Protein				NULL		0	NULL	NULL	NULL	gw60_molcell_3_1_77_s_93	10024881	(b) Binding of purified Eve proteins to GST-dTBP.	bind
8360	1	3674	6	11	NULL	NULL	NULL	Eve proteins	GP	purified	bind					GST-dTBP	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_10_3664_s_190	16672620	(B) Binding of purified Fur protein to the  ycgT regulatory region.	bind
8361	1	3674	6	11	NULL	NULL	NULL	Fur protein	GP	purified	bind					ycgT	GP			regulatory region	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_10_3664_s_190	16672620	(B) Binding of purified Fur protein to the  ycgT regulatory region.	bind
12096	1	3674	7	11	NULL	NULL	NULL	Fur protein	GP	purified	bind					ycgT	GP			regulatory region	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_10_3664_s_190	16672620	(B) Binding of purified Fur protein to the  ycgT regulatory region.	bind
81105	1	3674	11	NULL	NULL	0	NULL	Fur protein	Protein		binds to 					ycgT regulatory region	Protein				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_10_3664_s_190	16672620	(B) Binding of purified Fur protein to the  ycgT regulatory region.	bind
8362	1	3675	6	11	NULL	NULL	NULL	RGS4	GP	purified	bind					GST-beta''-COP	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_9_3155_s_136	10982407	(B) Binding of purified RGS4 to GST-beta''-COP.	bind
12097	1	3675	7	11	NULL	NULL	NULL	RGS4	GP	purified	bind					GST-beta''-COP	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_9_3155_s_136	10982407	(B) Binding of purified RGS4 to GST-beta''-COP.	bind
81106	1	3675	11	NULL	NULL	0	NULL	RGS4	Protein	purified	binds to 					GST-beta''-COP	Protein				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_9_3155_s_136	10982407	(B) Binding of purified RGS4 to GST-beta''-COP.	bind
8363	1	3676	6	11	NULL	NULL	NULL	DDR2-Fc	GP	radiolabelled	bind					cell surface	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_38	9659900	(B) Binding of radiolabelled DDR2-Fc to cell surfaces can be specifically competed by both DDR1 and DDR2 Rbodies (and not a control Rbody), demonstrating the specificity of binding and that both DDR receptors are binding to the same putative cell-associated ligand.	bind
8364	2	3676	6	11	NULL	NULL	NULL	DDR1 Rbodies	GP		bind					cell surface	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_38	9659900	(B) Binding of radiolabelled DDR2-Fc to cell surfaces can be specifically competed by both DDR1 and DDR2 Rbodies (and not a control Rbody), demonstrating the specificity of binding and that both DDR receptors are binding to the same putative cell-associated ligand.	bind
8366	3	3676	6	11	NULL	NULL	NULL	statement 1	Process		competes		specifically			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_38	9659900	(B) Binding of radiolabelled DDR2-Fc to cell surfaces can be specifically competed by both DDR1 and DDR2 Rbodies (and not a control Rbody), demonstrating the specificity of binding and that both DDR receptors are binding to the same putative cell-associated ligand.	bind
8367	4	3676	6	11	NULL	NULL	NULL	DDR2 Rbodies	GP		bind					cell surface	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_38	9659900	(B) Binding of radiolabelled DDR2-Fc to cell surfaces can be specifically competed by both DDR1 and DDR2 Rbodies (and not a control Rbody), demonstrating the specificity of binding and that both DDR receptors are binding to the same putative cell-associated ligand.	bind
8368	5	3676	6	11	NULL	NULL	NULL	statement 1	Process		competes		specifically			statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_38	9659900	(B) Binding of radiolabelled DDR2-Fc to cell surfaces can be specifically competed by both DDR1 and DDR2 Rbodies (and not a control Rbody), demonstrating the specificity of binding and that both DDR receptors are binding to the same putative cell-associated ligand.	bind
53027	6	3676	6	11	NULL	NULL	NULL	DDR receptors	GP		bind					cell-associated ligand	GP	putative			NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_38	9659900	(B) Binding of radiolabelled DDR2-Fc to cell surfaces can be specifically competed by both DDR1 and DDR2 Rbodies (and not a control Rbody), demonstrating the specificity of binding and that both DDR receptors are binding to the same putative cell-associated ligand.	bind
12100	2	3676	7	11	NULL	NULL	NULL	DDR1 Rbody 	GP		bind					cell surface  	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_38	9659900	(B) Binding of radiolabelled DDR2-Fc to cell surfaces can be specifically competed by both DDR1 and DDR2 Rbodies (and not a control Rbody), demonstrating the specificity of binding and that both DDR receptors are binding to the same putative cell-associated ligand.	bind
12101	3	3676	7	11	NULL	NULL	NULL	DDR2 Rbody	GP		bind					cell surface  	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_38	9659900	(B) Binding of radiolabelled DDR2-Fc to cell surfaces can be specifically competed by both DDR1 and DDR2 Rbodies (and not a control Rbody), demonstrating the specificity of binding and that both DDR receptors are binding to the same putative cell-associated ligand.	bind
12102	4	3676	7	11	NULL	NULL	NULL	statement 2	Process		compete with		specifically			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_38	9659900	(B) Binding of radiolabelled DDR2-Fc to cell surfaces can be specifically competed by both DDR1 and DDR2 Rbodies (and not a control Rbody), demonstrating the specificity of binding and that both DDR receptors are binding to the same putative cell-associated ligand.	bind
12103	5	3676	7	11	NULL	NULL	NULL	statement 3	Process		compete with		specifically			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_38	9659900	(B) Binding of radiolabelled DDR2-Fc to cell surfaces can be specifically competed by both DDR1 and DDR2 Rbodies (and not a control Rbody), demonstrating the specificity of binding and that both DDR receptors are binding to the same putative cell-associated ligand.	bind
12104	6	3676	7	11	NULL	NULL	NULL	DDR receptors	GP		bind					cell-associated ligand	GP	putative			NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_38	9659900	(B) Binding of radiolabelled DDR2-Fc to cell surfaces can be specifically competed by both DDR1 and DDR2 Rbodies (and not a control Rbody), demonstrating the specificity of binding and that both DDR receptors are binding to the same putative cell-associated ligand.	bind
81108	1	3676	11	NULL	NULL	0	NULL	DDR2-Fc	Protein	 radiolabelled	binds to 					cell surface	CellComponent				NULL		0	NULL	NULL	NULL	gw60_molcell_1_1_25_s_38	9659900	(B) Binding of radiolabelled DDR2-Fc to cell surfaces can be specifically competed by both DDR1 and DDR2 Rbodies (and not a control Rbody), demonstrating the specificity of binding and that both DDR receptors are binding to the same putative cell-associated ligand.	bind
81109	2	3676	11	NULL	NULL	0	NULL	DDR1 Rbodies	Protein		binds to 					cell surface	CellComponent				NULL		0	NULL	NULL	NULL	gw60_molcell_1_1_25_s_38	9659900	(B) Binding of radiolabelled DDR2-Fc to cell surfaces can be specifically competed by both DDR1 and DDR2 Rbodies (and not a control Rbody), demonstrating the specificity of binding and that both DDR receptors are binding to the same putative cell-associated ligand.	bind
81110	3	3676	11	NULL	NULL	0	NULL	DDR2 Rbodies	Protein		binds to 					cell surface	CellComponent				NULL		0	NULL	NULL	NULL	gw60_molcell_1_1_25_s_38	9659900	(B) Binding of radiolabelled DDR2-Fc to cell surfaces can be specifically competed by both DDR1 and DDR2 Rbodies (and not a control Rbody), demonstrating the specificity of binding and that both DDR receptors are binding to the same putative cell-associated ligand.	bind
81111	4	3676	11	NULL	NULL	0	NULL	DDR1 Rbodies	Protein		competes with					DDR2-Fc	Protein				NULL		0	NULL	NULL	NULL	gw60_molcell_1_1_25_s_38	9659900	(B) Binding of radiolabelled DDR2-Fc to cell surfaces can be specifically competed by both DDR1 and DDR2 Rbodies (and not a control Rbody), demonstrating the specificity of binding and that both DDR receptors are binding to the same putative cell-associated ligand.	bind
81112	5	3676	11	NULL	NULL	0	NULL	DDR2 Rbodies	Protein		competes with					DDR2-Fc	Protein				NULL		0	NULL	NULL	NULL	gw60_molcell_1_1_25_s_38	9659900	(B) Binding of radiolabelled DDR2-Fc to cell surfaces can be specifically competed by both DDR1 and DDR2 Rbodies (and not a control Rbody), demonstrating the specificity of binding and that both DDR receptors are binding to the same putative cell-associated ligand.	bind
81113	6	3676	11	NULL	NULL	0	NULL	DDR1 Rbodies	Protein		binds to 					cell-associated ligand	GeneOrProtein	putative 			NULL		0	NULL	NULL	NULL	gw60_molcell_1_1_25_s_38	9659900	(B) Binding of radiolabelled DDR2-Fc to cell surfaces can be specifically competed by both DDR1 and DDR2 Rbodies (and not a control Rbody), demonstrating the specificity of binding and that both DDR receptors are binding to the same putative cell-associated ligand.	bind
81114	7	3676	11	NULL	NULL	0	NULL	DDR2 Rbodies	Protein		binds to 					cell-associated ligand	GeneOrProtein	putative 			NULL		0	NULL	NULL	NULL	gw60_molcell_1_1_25_s_38	9659900	(B) Binding of radiolabelled DDR2-Fc to cell surfaces can be specifically competed by both DDR1 and DDR2 Rbodies (and not a control Rbody), demonstrating the specificity of binding and that both DDR receptors are binding to the same putative cell-associated ligand.	bind
8528	1	3677	6	11	NULL	NULL	NULL	elongin B 	GP	radiolabelled	bind					GST-elongin C	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_732_s_209	9447969	(B) Binding of radiolabelled elongin B to the indicated GST-elongin C fusion proteins (lanes 2 to 10).	bind
40916	2	3677	6	11	NULL	NULL	NULL	GST-elongin C	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_732_s_209	9447969	(B) Binding of radiolabelled elongin B to the indicated GST-elongin C fusion proteins (lanes 2 to 10).	bind
12106	1	3677	7	11	NULL	NULL	NULL	elongin B	GP	radiolabelled 	bind					GST-elongin C	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_732_s_209	9447969	(B) Binding of radiolabelled elongin B to the indicated GST-elongin C fusion proteins (lanes 2 to 10).	bind
53028	2	3677	7	11	NULL	NULL	NULL	GST-elongin C	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_732_s_209	9447969	(B) Binding of radiolabelled elongin B to the indicated GST-elongin C fusion proteins (lanes 2 to 10).	bind
81115	1	3677	11	NULL	NULL	0	NULL	elongin B	Protein	radiolabelled	binds to 					GST-elongin C fusion proteins	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_2_732_s_209	9447969	(B) Binding of radiolabelled elongin B to the indicated GST-elongin C fusion proteins (lanes 2 to 10).	bind
8529	1	3678	6	11	NULL	NULL	NULL	Raf-1	GP		bind					Rb	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7487_s_108	9819434	(B) Binding of Raf-1 to Rb and p130 but not to p107, E2F1, or DP proteins in a similar assay.	bind
8533	3	3678	6	11	NULL	NULL	NULL	Raf-1	GP		bind					p130	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7487_s_108	9819434	(B) Binding of Raf-1 to Rb and p130 but not to p107, E2F1, or DP proteins in a similar assay.	bind
8534	4	3678	6	11	NULL	NULL	NULL	Raf-1	GP		does not bind					p107	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7487_s_108	9819434	(B) Binding of Raf-1 to Rb and p130 but not to p107, E2F1, or DP proteins in a similar assay.	bind
8535	5	3678	6	11	NULL	NULL	NULL	Raf-1	GP		does not bind					E2F1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7487_s_108	9819434	(B) Binding of Raf-1 to Rb and p130 but not to p107, E2F1, or DP proteins in a similar assay.	bind
8536	6	3678	6	11	NULL	NULL	NULL	Raf-1	GP		does not bind					DP proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7487_s_108	9819434	(B) Binding of Raf-1 to Rb and p130 but not to p107, E2F1, or DP proteins in a similar assay.	bind
12099	1	3678	7	11	NULL	NULL	NULL	DDR2-Fc	GP	radiolabelled 	bind					cell surface  	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7487_s_108	9819434	(B) Binding of Raf-1 to Rb and p130 but not to p107, E2F1, or DP proteins in a similar assay.	bind
12107	1	3678	7	11	NULL	NULL	NULL	Raf-1	GP		bind					Rb	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7487_s_108	9819434	(B) Binding of Raf-1 to Rb and p130 but not to p107, E2F1, or DP proteins in a similar assay.	bind
12109	2	3678	7	11	NULL	NULL	NULL	Raf-1	GP		bind					p130	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7487_s_108	9819434	(B) Binding of Raf-1 to Rb and p130 but not to p107, E2F1, or DP proteins in a similar assay.	bind
12110	3	3678	7	11	NULL	NULL	NULL	Raf-1	GP		does not bind					p107	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7487_s_108	9819434	(B) Binding of Raf-1 to Rb and p130 but not to p107, E2F1, or DP proteins in a similar assay.	bind
12111	4	3678	7	11	NULL	NULL	NULL	Raf-1	GP		does not bind					E2F1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7487_s_108	9819434	(B) Binding of Raf-1 to Rb and p130 but not to p107, E2F1, or DP proteins in a similar assay.	bind
12112	5	3678	7	11	NULL	NULL	NULL	Raf-1	GP		does not bind					DP protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7487_s_108	9819434	(B) Binding of Raf-1 to Rb and p130 but not to p107, E2F1, or DP proteins in a similar assay.	bind
81116	1	3678	11	NULL	NULL	0	NULL	Raf-1	Protein		binds to 					Rb	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_12_7487_s_108	9819434	(B) Binding of Raf-1 to Rb and p130 but not to p107, E2F1, or DP proteins in a similar assay.	bind
81117	2	3678	11	NULL	NULL	0	NULL	Raf-1	Protein		binds to 					p130	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_12_7487_s_108	9819434	(B) Binding of Raf-1 to Rb and p130 but not to p107, E2F1, or DP proteins in a similar assay.	bind
81118	3	3678	11	NULL	NULL	NULL	NULL	Raf-1	Protein		does not bind to					p107 protein	Protein				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7487_s_108	9819434	(B) Binding of Raf-1 to Rb and p130 but not to p107, E2F1, or DP proteins in a similar assay.	bind
81119	4	3678	11	NULL	NULL	NULL	NULL	Raf-1	Protein		does not bind to					E2F1 protein	Protein				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7487_s_108	9819434	(B) Binding of Raf-1 to Rb and p130 but not to p107, E2F1, or DP proteins in a similar assay.	bind
81120	5	3678	11	NULL	NULL	0	NULL	Raf-1	Protein		does not bind to					DP protein	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_12_7487_s_108	9819434	(B) Binding of Raf-1 to Rb and p130 but not to p107, E2F1, or DP proteins in a similar assay.	bind
8540	1	3679	6	11	NULL	NULL	NULL	CBF3 proteins	GP	recombinant	bind					DNA	NucleicAcid			CDEIII 	NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_11_4557_s_108	13679521	(B) Binding of recombinant CBF3 proteins to CDEIII DNA (probe 2). "`	bind
12113	1	3679	7	11	NULL	NULL	NULL	CBF3 protein	GP	recombinant	bind					DNA	NucleicAcid			CDEIII 	NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_11_4557_s_108	13679521	(B) Binding of recombinant CBF3 proteins to CDEIII DNA (probe 2). "`	bind
81121	1	3679	11	NULL	NULL	0	NULL	CBF3 protein	Protein	 recombinant	binds to 					CDEIII DNA	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_11_4557_s_108	13679521	(B) Binding of recombinant CBF3 proteins to CDEIII DNA (probe 2). "`	bind
8543	1	3680	6	11	NULL	NULL	NULL	NF-I	GP	recombinant	bind			C220		UC	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_72_1_65_s_137	10521600	(B) Binding of recombinant NF-I C220 to UC, UCY and UBE.	bind
8546	2	3680	6	11	NULL	NULL	NULL	NF-I	GP	recombinant	bind			C220		UCY	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_72_1_65_s_137	10521600	(B) Binding of recombinant NF-I C220 to UC, UCY and UBE.	bind
8547	3	3680	6	11	NULL	NULL	NULL	NF-I	GP	recombinant	bind			C220		UBE	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_72_1_65_s_137	10521600	(B) Binding of recombinant NF-I C220 to UC, UCY and UBE.	bind
12114	1	3680	7	11	NULL	NULL	NULL	NF-I 	GP	recombinant	bind			C220 		UC	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_72_1_65_s_137	10521600	(B) Binding of recombinant NF-I C220 to UC, UCY and UBE.	bind
12115	2	3680	7	11	NULL	NULL	NULL	NF-I 	GP	recombinant	bind			C220 		UCY	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_72_1_65_s_137	10521600	(B) Binding of recombinant NF-I C220 to UC, UCY and UBE.	bind
12116	3	3680	7	11	NULL	NULL	NULL	NF-I	GP	recombinant	bind			C220		UBE	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_72_1_65_s_137	10521600	(B) Binding of recombinant NF-I C220 to UC, UCY and UBE.	bind
81217	1	3680	11	NULL	NULL	0	NULL	NF-I C220	Protein		binds to 					UC	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_brainresmolbrainres_72_1_65_s_137	10521600	(B) Binding of recombinant NF-I C220 to UC, UCY and UBE.	bind
81218	2	3680	11	NULL	NULL	0	NULL	NF-I C220	Protein		binds to 					UCY	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_brainresmolbrainres_72_1_65_s_137	10521600	(B) Binding of recombinant NF-I C220 to UC, UCY and UBE.	bind
81219	3	3680	11	NULL	NULL	NULL	NULL	NF-I C220	Protein		binds to 					UBE	NucleicAcidSubstance				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_72_1_65_s_137	10521600	(B) Binding of recombinant NF-I C220 to UC, UCY and UBE.	bind
8552	1	3681	6	11	NULL	NULL	NULL	SP-1	GP	recombinant	bind					TK-SP1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8442_s_188	10567569	(B) Binding of recombinant SP-1 to a TK-SP1 or to the indicated E2F elements.	bind
8558	2	3681	6	11	NULL	NULL	NULL	SP-1	GP	recombinant	bind									E2F element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8442_s_188	10567569	(B) Binding of recombinant SP-1 to a TK-SP1 or to the indicated E2F elements.	bind
40923	3	3681	6	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8442_s_188	10567569	(B) Binding of recombinant SP-1 to a TK-SP1 or to the indicated E2F elements.	bind
12117	1	3681	7	11	NULL	NULL	NULL	SP-1	GP	recombinant	bind					TK-SP1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8442_s_188	10567569	(B) Binding of recombinant SP-1 to a TK-SP1 or to the indicated E2F elements.	bind
12118	2	3681	7	11	NULL	NULL	NULL	SP-1	GP	recombinant	bind									E2F element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8442_s_188	10567569	(B) Binding of recombinant SP-1 to a TK-SP1 or to the indicated E2F elements.	bind
12119	3	3681	7	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8442_s_188	10567569	(B) Binding of recombinant SP-1 to a TK-SP1 or to the indicated E2F elements.	bind
81220	1	3681	11	NULL	NULL	0	NULL	SP-1	Protein		binds to 					TK-SP1 	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_12_8442_s_188	10567569	(B) Binding of recombinant SP-1 to a TK-SP1 or to the indicated E2F elements.	bind
81221	2	3681	11	NULL	NULL	0	NULL	SP-1	Protein		binds to 					E2F	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_12_8442_s_188	10567569	(B) Binding of recombinant SP-1 to a TK-SP1 or to the indicated E2F elements.	bind
8559	1	3682	6	11	NULL	NULL	NULL	RPA	GP		bind					p53	GP			UV lesions	NULL	HEK293T cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_39_s_95	16354678	(B) Binding of RPA to UV and  N-AAAF lesions in the p53 of HEK293T cells.	bind
8560	2	3682	6	11	NULL	NULL	NULL	RPA	GP		bind					p53	GP			N-AAAF lesions	NULL	HEK293T cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_39_s_95	16354678	(B) Binding of RPA to UV and  N-AAAF lesions in the p53 of HEK293T cells.	bind
12120	1	3682	7	11	NULL	NULL	NULL	RPA	GP		bind					p53	GP			UV lesion 	NULL	HEK293T cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_39_s_95	16354678	(B) Binding of RPA to UV and  N-AAAF lesions in the p53 of HEK293T cells.	bind
12121	2	3682	7	11	NULL	NULL	NULL	RPA	GP		bind					p53	GP			N-AAAF lesion	NULL	HEK293T cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_39_s_95	16354678	(B) Binding of RPA to UV and  N-AAAF lesions in the p53 of HEK293T cells.	bind
81222	1	3682	11	NULL	NULL	0	NULL	UV	EnvironmentalFactor		makes lesions in					p53	Protein	HEK293T cells			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_1_39_s_95	16354678	(B) Binding of RPA to UV and  N-AAAF lesions in the p53 of HEK293T cells.	bind
81223	2	3682	11	NULL	NULL	0	NULL	N-AAAF	Chemical		makes lesions in					p53	Protein	HEK293T cells			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_1_39_s_95	16354678	(B) Binding of RPA to UV and  N-AAAF lesions in the p53 of HEK293T cells.	bind
81224	3	3682	11	NULL	NULL	0	NULL	RPA	Protein		binds to 					statement 1	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_1_39_s_95	16354678	(B) Binding of RPA to UV and  N-AAAF lesions in the p53 of HEK293T cells.	bind
81225	4	3682	11	NULL	NULL	0	NULL	RPA	Protein		binds to 					statement 2	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_1_39_s_95	16354678	(B) Binding of RPA to UV and  N-AAAF lesions in the p53 of HEK293T cells.	bind
8561	1	3683	6	11	NULL	NULL	NULL	Skp1	GP		bind					Skp2	GP	truncation mutant			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_635_s_169	9858587	(B) Binding of Skp1 and cyclin A-Cdk2 to Skp2 truncation mutants.	bind
8562	2	3683	6	11	NULL	NULL	NULL	cyclin A-Cdk2	GP		bind					Skp2	GP	truncation mutant			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_635_s_169	9858587	(B) Binding of Skp1 and cyclin A-Cdk2 to Skp2 truncation mutants.	bind
12122	1	3683	7	11	NULL	NULL	NULL	Skp1	GP		bind					Skp2	GP	truncation mutant			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_635_s_169	9858587	(B) Binding of Skp1 and cyclin A-Cdk2 to Skp2 truncation mutants.	bind
12123	2	3683	7	11	NULL	NULL	NULL	cyclin A-Cdk2	GP		bind					Skp2	GP	truncation mutant			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_635_s_169	9858587	(B) Binding of Skp1 and cyclin A-Cdk2 to Skp2 truncation mutants.	bind
81226	1	3683	11	NULL	NULL	0	NULL	Skp1	Protein		binds to 					Skp2 mutants	Protein	truncation			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_1_635_s_169	9858587	(B) Binding of Skp1 and cyclin A-Cdk2 to Skp2 truncation mutants.	bind
81227	2	3683	11	NULL	NULL	0	NULL	cyclin A-Cdk2	Protein		binds to 					Skp2 mutants	Protein	truncation			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_1_635_s_169	9858587	(B) Binding of Skp1 and cyclin A-Cdk2 to Skp2 truncation mutants.	bind
8563	1	3684	6	11	NULL	NULL	NULL	Skp2	GP		bind					cyclin D2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_5_1189_s_257	12769844	(B) Binding of Skp2, Sug1, and Ub to the cyclin D2 promoter is Myc dependent.	bind
8564	2	3684	6	11	NULL	NULL	NULL	Sug1	GP		bind					cyclin D2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_5_1189_s_257	12769844	(B) Binding of Skp2, Sug1, and Ub to the cyclin D2 promoter is Myc dependent.	bind
8565	3	3684	6	11	NULL	NULL	NULL	Ub	GP		bind					cyclin D2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_5_1189_s_257	12769844	(B) Binding of Skp2, Sug1, and Ub to the cyclin D2 promoter is Myc dependent.	bind
8566	4	3684	6	11	NULL	NULL	NULL	statement 1	Process		is dependent on					Myc	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_5_1189_s_257	12769844	(B) Binding of Skp2, Sug1, and Ub to the cyclin D2 promoter is Myc dependent.	bind
8567	5	3684	6	11	NULL	NULL	NULL	statement 2	Process		is dependent on					Myc	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_5_1189_s_257	12769844	(B) Binding of Skp2, Sug1, and Ub to the cyclin D2 promoter is Myc dependent.	bind
8568	6	3684	6	11	NULL	NULL	NULL	statement 3	Process		is dependent on					Myc	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_5_1189_s_257	12769844	(B) Binding of Skp2, Sug1, and Ub to the cyclin D2 promoter is Myc dependent.	bind
12124	1	3684	7	11	NULL	NULL	NULL	Skp2	GP		bind					cyclin D2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_5_1189_s_257	12769844	(B) Binding of Skp2, Sug1, and Ub to the cyclin D2 promoter is Myc dependent.	bind
12125	2	3684	7	11	NULL	NULL	NULL	Sug1	GP		bind					cyclin D2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_5_1189_s_257	12769844	(B) Binding of Skp2, Sug1, and Ub to the cyclin D2 promoter is Myc dependent.	bind
12126	3	3684	7	11	NULL	NULL	NULL	Ub	GP		bind					cyclin D2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_5_1189_s_257	12769844	(B) Binding of Skp2, Sug1, and Ub to the cyclin D2 promoter is Myc dependent.	bind
12127	4	3684	7	11	NULL	NULL	NULL	statement 1	Process		is dependent on					Myc	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_5_1189_s_257	12769844	(B) Binding of Skp2, Sug1, and Ub to the cyclin D2 promoter is Myc dependent.	bind
12128	5	3684	7	11	NULL	NULL	NULL	statement 2	Process		is dependent on					Myc	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_5_1189_s_257	12769844	(B) Binding of Skp2, Sug1, and Ub to the cyclin D2 promoter is Myc dependent.	bind
12129	6	3684	7	11	NULL	NULL	NULL	statement 3	Process		is dependent on					Myc	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_5_1189_s_257	12769844	(B) Binding of Skp2, Sug1, and Ub to the cyclin D2 promoter is Myc dependent.	bind
81228	1	3684	11	NULL	NULL	0	NULL	Skp2	Protein		binds to 					cyclin D2 promoter	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcell_11_5_1189_s_257	12769844	(B) Binding of Skp2, Sug1, and Ub to the cyclin D2 promoter is Myc dependent.	bind
81229	2	3684	11	NULL	NULL	0	NULL	Sug1	Protein		binds to 					cyclin D2 promoter	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcell_11_5_1189_s_257	12769844	(B) Binding of Skp2, Sug1, and Ub to the cyclin D2 promoter is Myc dependent.	bind
81230	3	3684	11	NULL	NULL	0	NULL	Ub	Protein		binds to 					cyclin D2 promoter	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcell_11_5_1189_s_257	12769844	(B) Binding of Skp2, Sug1, and Ub to the cyclin D2 promoter is Myc dependent.	bind
81231	4	3684	11	NULL	NULL	0	NULL	statement 1	Process		depends on					Myc	Protein				NULL		0	NULL	NULL	NULL	gw60_molcell_11_5_1189_s_257	12769844	(B) Binding of Skp2, Sug1, and Ub to the cyclin D2 promoter is Myc dependent.	bind
81232	5	3684	11	NULL	NULL	0	NULL	statement 2	Process		depends on					Myc	Protein				NULL		0	NULL	NULL	NULL	gw60_molcell_11_5_1189_s_257	12769844	(B) Binding of Skp2, Sug1, and Ub to the cyclin D2 promoter is Myc dependent.	bind
81233	6	3684	11	NULL	NULL	0	NULL	statement 3	Process		depends on					Myc	Protein				NULL		0	NULL	NULL	NULL	gw60_molcell_11_5_1189_s_257	12769844	(B) Binding of Skp2, Sug1, and Ub to the cyclin D2 promoter is Myc dependent.	bind
8569	1	3685	6	11	NULL	NULL	NULL	bHA	GP	soluble	bind					layilin-IgG	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_891_s_168	11294894	(B) Binding of soluble bHA to layilin-IgG (L-IgG) or CD44-IgG immobilized in microtiter wells.	bind
8570	2	3685	6	11	NULL	NULL	NULL	bHA	GP	soluble	bind					CD44-IgG	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_891_s_168	11294894	(B) Binding of soluble bHA to layilin-IgG (L-IgG) or CD44-IgG immobilized in microtiter wells.	bind
8571	3	3685	6	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_891_s_168	11294894	(B) Binding of soluble bHA to layilin-IgG (L-IgG) or CD44-IgG immobilized in microtiter wells.	bind
40936	4	3685	6	11	NULL	NULL	NULL	L-IgG	GP		is					layilin-IgG	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_891_s_168	11294894	(B) Binding of soluble bHA to layilin-IgG (L-IgG) or CD44-IgG immobilized in microtiter wells.	bind
12130	1	3685	7	11	NULL	NULL	NULL	bHA	GP	soluble	bind					layilin-IgG	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_891_s_168	11294894	(B) Binding of soluble bHA to layilin-IgG (L-IgG) or CD44-IgG immobilized in microtiter wells.	bind
12131	2	3685	7	11	NULL	NULL	NULL	bHA	GP	soluble	bind					CD44-IgG	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_891_s_168	11294894	(B) Binding of soluble bHA to layilin-IgG (L-IgG) or CD44-IgG immobilized in microtiter wells.	bind
12132	3	3685	7	11	NULL	NULL	NULL	layilin-IgG	GP		is					L-IgG	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_891_s_168	11294894	(B) Binding of soluble bHA to layilin-IgG (L-IgG) or CD44-IgG immobilized in microtiter wells.	bind
12133	4	3685	7	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_4_891_s_168	11294894	(B) Binding of soluble bHA to layilin-IgG (L-IgG) or CD44-IgG immobilized in microtiter wells.	bind
81234	1	3685	11	NULL	NULL	0	NULL	layilin-IgG	PartOfProtein		is					L-IgG	PartOfProtein				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_4_891_s_168	11294894	(B) Binding of soluble bHA to layilin-IgG (L-IgG) or CD44-IgG immobilized in microtiter wells.	bind
81235	2	3685	11	NULL	NULL	0	NULL	bHA	NonProteinOrNucleicAcidChemical	soluble	binds to 					layilin-IgG	PartOfProtein				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_4_891_s_168	11294894	(B) Binding of soluble bHA to layilin-IgG (L-IgG) or CD44-IgG immobilized in microtiter wells.	bind
81236	3	3685	11	NULL	NULL	0	NULL	bHA	NonProteinOrNucleicAcidChemical	soluble	binds to 					CD44-IgG	PartOfProtein				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_4_891_s_168	11294894	(B) Binding of soluble bHA to layilin-IgG (L-IgG) or CD44-IgG immobilized in microtiter wells.	bind
8572	1	3686	6	11	NULL	NULL	NULL	Sp1	GP		bind									TSA-response element	NULL	Hep3B cells	NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_4_1005_s_114	12200149	(B) Binding of Sp1 and Sp3 to the TSA-response element in Hep3B cells.	bind
8573	2	3686	6	11	NULL	NULL	NULL	Sp3	GP		bind									TSA-response element	NULL	Hep3B cells	NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_4_1005_s_114	12200149	(B) Binding of Sp1 and Sp3 to the TSA-response element in Hep3B cells.	bind
12134	1	3686	7	11	NULL	NULL	NULL	Sp1 	GP		bind									TSA-response element	NULL	Hep3B cells	NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_4_1005_s_114	12200149	(B) Binding of Sp1 and Sp3 to the TSA-response element in Hep3B cells.	bind
12135	2	3686	7	11	NULL	NULL	NULL	Sp3	GP		bind									TSA-response element	NULL	Hep3B cells	NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_4_1005_s_114	12200149	(B) Binding of Sp1 and Sp3 to the TSA-response element in Hep3B cells.	bind
81237	1	3686	11	NULL	NULL	0	NULL	Sp1	Protein		binds to 					TSA-response element	NucleicAcidSubstance	Hep3B cells			NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_4_1005_s_114	12200149	(B) Binding of Sp1 and Sp3 to the TSA-response element in Hep3B cells.	bind
81238	2	3686	11	NULL	NULL	0	NULL	Sp3	Protein		binds to 					TSA-response element	NucleicAcidSubstance	Hep3B cells			NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_4_1005_s_114	12200149	(B) Binding of Sp1 and Sp3 to the TSA-response element in Hep3B cells.	bind
8574	1	3687	6	11	NULL	NULL	NULL	sperm cells	Cell		bind					zona pellucida	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_267_1_203_s_232	14975727	(B) Binding of sperm cells to the zona pellucida.	bind
12136	1	3687	7	11	NULL	NULL	NULL	sperm cells	Cell		bind					zona pellucida	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_267_1_203_s_232	14975727	(B) Binding of sperm cells to the zona pellucida.	bind
81239	1	3687	11	NULL	NULL	0	NULL	sperm cells	cell		binds to 					zona pellucida	AnatomicalPart				NULL		0	NULL	NULL	NULL	gw70_devbiol_267_1_203_s_232	14975727	(B) Binding of sperm cells to the zona pellucida.	bind
8575	1	3688	6	11	NULL	NULL	NULL	syncollin	GP		bind					GST-syntaxin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_90_2_325_s_135	9244306	(B) Binding of syncollin to GST-syntaxin in  the presence of 1 mM EGTA or 100 muM free Ca2+.	bind
8576	2	3688	6	11	NULL	NULL	NULL	statement 1	Process		occurs in presence of					EGTA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_90_2_325_s_135	9244306	(B) Binding of syncollin to GST-syntaxin in  the presence of 1 mM EGTA or 100 muM free Ca2+.	bind
8577	3	3688	6	11	NULL	NULL	NULL	statement 1	Process		occurs in presence of					Ca+2	Chemical	free			NULL		NULL	NULL	NULL	NULL	gw60_cell_90_2_325_s_135	9244306	(B) Binding of syncollin to GST-syntaxin in  the presence of 1 mM EGTA or 100 muM free Ca2+.	bind
53029	4	3688	6	11	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_90_2_325_s_135	9244306	(B) Binding of syncollin to GST-syntaxin in  the presence of 1 mM EGTA or 100 muM free Ca2+.	bind
12137	1	3688	7	11	NULL	NULL	NULL	syncollin 	GP		bind					GST-syntaxin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_90_2_325_s_135	9244306	(B) Binding of syncollin to GST-syntaxin in  the presence of 1 mM EGTA or 100 muM free Ca2+.	bind
44731	3	3688	7	11	NULL	NULL	NULL	statement 1	GP		in the presence of					EGTA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_90_2_325_s_135	9244306	(B) Binding of syncollin to GST-syntaxin in  the presence of 1 mM EGTA or 100 muM free Ca2+.	bind
44732	2	3688	7	11	NULL	NULL	NULL	statement 1	Process		in the presence of 					free Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_90_2_325_s_135	9244306	(B) Binding of syncollin to GST-syntaxin in  the presence of 1 mM EGTA or 100 muM free Ca2+.	bind
44733	4	3688	7	11	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_90_2_325_s_135	9244306	(B) Binding of syncollin to GST-syntaxin in  the presence of 1 mM EGTA or 100 muM free Ca2+.	bind
81240	1	3688	11	NULL	NULL	0	NULL	syncollin	Protein		binds to 					GST-syntaxin	Protein				NULL		0	NULL	NULL	NULL	gw60_cell_90_2_325_s_135	9244306	(B) Binding of syncollin to GST-syntaxin in  the presence of 1 mM EGTA or 100 muM free Ca2+.	bind
81241	2	3688	11	NULL	NULL	0	NULL	statement 1	Process		occurs in the presence of					EGTA	Chemical				NULL		0	NULL	NULL	NULL	gw60_cell_90_2_325_s_135	9244306	(B) Binding of syncollin to GST-syntaxin in  the presence of 1 mM EGTA or 100 muM free Ca2+.	bind
81242	3	3688	11	NULL	NULL	0	NULL	statement 1	Process		occurs in the presence of					free Ca2+	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	gw60_cell_90_2_325_s_135	9244306	(B) Binding of syncollin to GST-syntaxin in  the presence of 1 mM EGTA or 100 muM free Ca2+.	bind
8578	1	3689	6	11	NULL	NULL	NULL	TBL1	GP		bind					H4	GP	biotinylated	tail peptide		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_1_324_s_82	15601853	(B) Binding of TBL1 and TBLR1 to a biotinylated H4 tail peptide  with or without acetylation on lysines 5, 8, 12, and 16.	bind
8579	2	3689	6	11	NULL	NULL	NULL	TBLR1	GP		bind					H4 	GP	biotinylated	tail peptide		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_1_324_s_82	15601853	(B) Binding of TBL1 and TBLR1 to a biotinylated H4 tail peptide  with or without acetylation on lysines 5, 8, 12, and 16.	bind
12140	1	3689	7	11	NULL	NULL	NULL	TBL1	GP		bind					H4	GP	biotinylated	tail peptide		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_1_324_s_82	15601853	(B) Binding of TBL1 and TBLR1 to a biotinylated H4 tail peptide  with or without acetylation on lysines 5, 8, 12, and 16.	bind
12142	2	3689	7	11	NULL	NULL	NULL	TBLR1	GP		bind					H4	GP	biotinylated	tail peptide		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_1_324_s_82	15601853	(B) Binding of TBL1 and TBLR1 to a biotinylated H4 tail peptide  with or without acetylation on lysines 5, 8, 12, and 16.	bind
81243	1	3689	11	NULL	NULL	0	NULL	TBL1	Protein		binds to 					H4 tail peptide	PartOfProtein	biotinylated			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_1_324_s_82	15601853	(B) Binding of TBL1 and TBLR1 to a biotinylated H4 tail peptide  with or without acetylation on lysines 5, 8, 12, and 16.	bind
81244	2	3689	11	NULL	NULL	0	NULL	TBLR1	Protein		binds to 					H4 tail peptide	PartOfProtein	biotinylated			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_1_324_s_82	15601853	(B) Binding of TBL1 and TBLR1 to a biotinylated H4 tail peptide  with or without acetylation on lysines 5, 8, 12, and 16.	bind
81245	3	3689	11	NULL	NULL	0	NULL	statement 1	Process		is independent of					lysines	AminoAcid	acetylation			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_1_324_s_82	15601853	(B) Binding of TBL1 and TBLR1 to a biotinylated H4 tail peptide  with or without acetylation on lysines 5, 8, 12, and 16.	bind
8580	1	3690	6	11	NULL	NULL	NULL	BAZF	GP		bind					Bcl6	GP		1-520		NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_303_2_600_s_121	12659862	(B) Binding of the 27  aa of BAZF to Bcl6(1-520) by the pull-down assay.	bind
12151	1	3690	7	11	NULL	NULL	NULL	BAZF	GP		bind					Bcl6	GP		1-520		NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_303_2_600_s_121	12659862	(B) Binding of the 27  aa of BAZF to Bcl6(1-520) by the pull-down assay.	bind
81246	1	3690	11	NULL	NULL	0	NULL	27 aa	AminoAcid	BAZF	binds to 					Bcl6	Protein				NULL	 pull-down assay	0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_303_2_600_s_121	12659862	(B) Binding of the 27  aa of BAZF to Bcl6(1-520) by the pull-down assay.	bind
8581	1	3691	6	11	NULL	NULL	NULL	Abl	GP		bind			SH3 domain		proline-rich sequences	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_152_s_201	9418863	(B) Binding of the Abl SH3 domain to proline-rich sequences is not required for phosphorylation of Ena.	bind
8585	2	3691	6	11	NULL	NULL	NULL	statement 1	Process		is not required for					Ena	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_152_s_201	9418863	(B) Binding of the Abl SH3 domain to proline-rich sequences is not required for phosphorylation of Ena.	bind
12152	1	3691	7	11	NULL	NULL	NULL	Abl	GP		bind			SH3 domain		proline-rich sequence	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_152_s_201	9418863	(B) Binding of the Abl SH3 domain to proline-rich sequences is not required for phosphorylation of Ena.	bind
12153	2	3691	7	11	NULL	NULL	NULL	statement 1	Process		is not required for					Ena	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_152_s_201	9418863	(B) Binding of the Abl SH3 domain to proline-rich sequences is not required for phosphorylation of Ena.	bind
81247	1	3691	11	NULL	NULL	0	NULL	Abl	Protein	SH3 domain	binds to 					proline-rich sequence	PartOfProtein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_152_s_201	9418863	(B) Binding of the Abl SH3 domain to proline-rich sequences is not required for phosphorylation of Ena.	bind
81248	2	3691	11	NULL	NULL	0	NULL	Ena	Protein		undergoes					phosphorylation	MolecularProcess				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_152_s_201	9418863	(B) Binding of the Abl SH3 domain to proline-rich sequences is not required for phosphorylation of Ena.	bind
81249	3	3691	11	NULL	NULL	0	NULL	statement 1	Process		is not required for					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_152_s_201	9418863	(B) Binding of the Abl SH3 domain to proline-rich sequences is not required for phosphorylation of Ena.	bind
8595	1	3692	6	11	NULL	NULL	NULL	CED-4	GP	mutant	bind					E1B 19K	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_10_6052_s_213	9742122	(B) Binding of the CED-4 mutant proteins to E1B 19K.	bind
12154	1	3692	7	11	NULL	NULL	NULL	CED-4	GP	mutant	bind					E1B 19K	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_10_6052_s_213	9742122	(B) Binding of the CED-4 mutant proteins to E1B 19K.	bind
81250	1	3692	11	NULL	NULL	0	NULL	CED-4 proteins	Protein	mutant 	binds to 					E1B 19K	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_10_6052_s_213	9742122	(B) Binding of the CED-4 mutant proteins to E1B 19K.	bind
8599	1	3693	6	11	NULL	NULL	NULL	HAP1-PPR1	GP		bind					UAS1/ CYC1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_3819_s_312	9632766	(B) Binding of the HAP1-PPR1 hybrid protein to UAS1/ CYC1 and UAS/ CYC7.	bind
8602	2	3693	6	11	NULL	NULL	NULL	HAP1-PPR1	GP		bind					UAS/CYC7	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_3819_s_312	9632766	(B) Binding of the HAP1-PPR1 hybrid protein to UAS1/ CYC1 and UAS/ CYC7.	bind
40942	3	3693	6	11	NULL	NULL	NULL	HAP1-PPR1	GP		is a type of					hybrid protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_3819_s_312	9632766	(B) Binding of the HAP1-PPR1 hybrid protein to UAS1/ CYC1 and UAS/ CYC7.	bind
12155	1	3693	7	11	NULL	NULL	NULL	HAP1-PPR1	GP		bind					UAS1/ CYC1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_3819_s_312	9632766	(B) Binding of the HAP1-PPR1 hybrid protein to UAS1/ CYC1 and UAS/ CYC7.	bind
12156	2	3693	7	11	NULL	NULL	NULL	HAP1-PPR1 	GP		bind					UAS/ CYC7	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_3819_s_312	9632766	(B) Binding of the HAP1-PPR1 hybrid protein to UAS1/ CYC1 and UAS/ CYC7.	bind
53030	3	3693	7	11	NULL	NULL	NULL	HAP1-PPR1	GP		is a type of					hybrid protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_3819_s_312	9632766	(B) Binding of the HAP1-PPR1 hybrid protein to UAS1/ CYC1 and UAS/ CYC7.	bind
81251	1	3693	11	NULL	NULL	0	NULL	HAP1-PPR1 hybrid protein	Protein		binds to 					 UAS1/ CYC1	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_7_3819_s_312	9632766	(B) Binding of the HAP1-PPR1 hybrid protein to UAS1/ CYC1 and UAS/ CYC7.	bind
81252	2	3693	11	NULL	NULL	0	NULL	HAP1-PPR1 hybrid protein	Protein		binds to 					UAS/ CYC7	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_7_3819_s_312	9632766	(B) Binding of the HAP1-PPR1 hybrid protein to UAS1/ CYC1 and UAS/ CYC7.	bind
8605	1	3694	6	11	NULL	NULL	NULL	p120 E4F protein	GP	purified	bind					Cyclin A	GP			CRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_8_2956_s_227	11283272	(B) Binding of the purified p120 E4F protein to cyclin A CRE.	bind
12157	1	3694	7	11	NULL	NULL	NULL	p120 E4F protein	GP	purified	bind					cyclin A	GP			CRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_8_2956_s_227	11283272	(B) Binding of the purified p120 E4F protein to cyclin A CRE.	bind
81253	1	3694	11	NULL	NULL	0	NULL	p120 E4F protein	Protein	purified	binds to 					cyclin A CRE	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_8_2956_s_227	11283272	(B) Binding of the purified p120 E4F protein to cyclin A CRE.	bind
8607	1	3695	6	11	NULL	NULL	NULL	Pax6 isoforms	GP		bind					F-crystallin	GP			enhancer	NULL		NULL	NULL	NULL	NULL	gw60_gene_286_2_271_s_108	11943482	(B) Binding of the two Pax6 isoforms to the  F-crystallin enhancer.	bind
12158	1	3695	7	11	NULL	NULL	NULL	Pax6 isoform	GP		bind					F-crystallin	GP			enhancer	NULL		NULL	NULL	NULL	NULL	gw60_gene_286_2_271_s_108	11943482	(B) Binding of the two Pax6 isoforms to the  F-crystallin enhancer.	bind
81338	1	3695	11	NULL	NULL	0	NULL	Pax6	Protein		binds to 					F-crystallin enhancer	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_gene_286_2_271_s_108	11943482	(B) Binding of the two Pax6 isoforms to the  F-crystallin enhancer.	bind
12159	1	3696	7	11	NULL	NULL	NULL	TIE2 receptor	GP		bind					Angiopoietin-1	GP	cloned			NULL		NULL	NULL	NULL	NULL	gw60_cell_87_7_1161_s_100	8980223	(B) Binding of TIE2 receptors by cloned  Angiopoietin-1.	bind
81339	1	3696	11	NULL	NULL	0	NULL	TIE2 receptors	GeneOrProtein		binds to 					Angiopoietin-1	GeneOrProtein	cloned			NULL		0	NULL	NULL	NULL	gw60_cell_87_7_1161_s_100	8980223	(B) Binding of TIE2 receptors by cloned  Angiopoietin-1.	bind
8611	1	3697	6	11	NULL	NULL	NULL	TIE2 receptors	GP		bind					Angiopoietin-1	GP	cloned			NULL		NULL	NULL	NULL	NULL	gw60_neuron_20_5_905_s_109	9620695	(B) Binding of tomosyn to truncated forms of syntaxin-1a.	bind
8618	1	3697	6	11	NULL	NULL	NULL	tomosyn	GP		bind					syntaxin-1A	GP	truncated forms of 			NULL		NULL	NULL	NULL	NULL	gw60_neuron_20_5_905_s_109	9620695	(B) Binding of tomosyn to truncated forms of syntaxin-1a.	bind
12160	1	3697	7	11	NULL	NULL	NULL	tomosyn	GP		bind					syntaxin-1a	GP	truncated forms of			NULL		NULL	NULL	NULL	NULL	gw60_neuron_20_5_905_s_109	9620695	(B) Binding of tomosyn to truncated forms of syntaxin-1a.	bind
81341	1	3697	11	NULL	NULL	0	NULL	tomosyn	GeneOrProtein		binds to 					syntaxin-1a	GeneOrProtein	 truncated			NULL		0	NULL	NULL	NULL	gw60_neuron_20_5_905_s_109	9620695	(B) Binding of tomosyn to truncated forms of syntaxin-1a.	bind
8619	1	3698	6	11	NULL	NULL	NULL	v-Src	GP		bind					His6Cdc37	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_6_1051_s_89	12499358	(B) Binding of v-Src and Hsp90 to human His6Cdc37 and His6Cdc371 - 173.	bind
8620	2	3698	6	11	NULL	NULL	NULL	Hsp90	GP		bind					His6Cdc37	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_6_1051_s_89	12499358	(B) Binding of v-Src and Hsp90 to human His6Cdc37 and His6Cdc371 - 173.	bind
8621	2	3698	6	11	NULL	NULL	NULL	v-Src	GP		bind					His6Cdc37	GP	human	1 - 173		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_6_1051_s_89	12499358	(B) Binding of v-Src and Hsp90 to human His6Cdc37 and His6Cdc371 - 173.	bind
8622	4	3698	6	11	NULL	NULL	NULL	Hsp90	GP		bind					His6Cdc37	GP	human	1 - 173		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_6_1051_s_89	12499358	(B) Binding of v-Src and Hsp90 to human His6Cdc37 and His6Cdc371 - 173.	bind
12161	1	3698	7	11	NULL	NULL	NULL	v-Src	GP		bind					His6Cdc37	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_6_1051_s_89	12499358	(B) Binding of v-Src and Hsp90 to human His6Cdc37 and His6Cdc371 - 173.	bind
12162	2	3698	7	11	NULL	NULL	NULL	v-Src	GP		bind					His6Cdc37	GP	human	1-173		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_6_1051_s_89	12499358	(B) Binding of v-Src and Hsp90 to human His6Cdc37 and His6Cdc371 - 173.	bind
12163	3	3698	7	11	NULL	NULL	NULL	Hsp90	GP		bind					His6Cdc37	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_6_1051_s_89	12499358	(B) Binding of v-Src and Hsp90 to human His6Cdc37 and His6Cdc371 - 173.	bind
12164	4	3698	7	11	NULL	NULL	NULL	Hsp90	GP		bind					His6Cdc37	GP	human	1-173		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_6_1051_s_89	12499358	(B) Binding of v-Src and Hsp90 to human His6Cdc37 and His6Cdc371 - 173.	bind
81359	1	3698	11	NULL	NULL	NULL	NULL	 v-Src	GeneOrProtein		binds to 					Cdc37	Protein	human	His6		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_6_1051_s_89	12499358	(B) Binding of v-Src and Hsp90 to human His6Cdc37 and His6Cdc371 - 173.	bind
81360	2	3698	11	NULL	NULL	0	NULL	Hsp90	GeneOrProtein		binds to 					Cdc37	Protein	human	His6		NULL		0	NULL	NULL	NULL	gw60_cellbiol_159_6_1051_s_89	12499358	(B) Binding of v-Src and Hsp90 to human His6Cdc37 and His6Cdc371 - 173.	bind
8769	1	3699	6	11	NULL	NULL	NULL	Vav	GP		bind					GST-hSiah2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3798_s_132	10207103	(B) Binding of Vav to GST-hSiah2 fusion proteins.	bind
40946	2	3699	6	11	NULL	NULL	NULL	GST-hSiah2	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3798_s_132	10207103	(B) Binding of Vav to GST-hSiah2 fusion proteins.	bind
12165	1	3699	7	11	NULL	NULL	NULL	Vav	GP		bind					 GST-hSiah2 	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3798_s_132	10207103	(B) Binding of Vav to GST-hSiah2 fusion proteins.	bind
44771	2	3699	7	11	NULL	NULL	NULL	GST-hSiah2	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3798_s_132	10207103	(B) Binding of Vav to GST-hSiah2 fusion proteins.	bind
81361	1	3699	11	NULL	NULL	0	NULL	Vav	Protein		binds to 					GST-hSiah2 	Protein	fusion protein			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3798_s_132	10207103	(B) Binding of Vav to GST-hSiah2 fusion proteins.	bind
8770	1	3700	6	11	NULL	NULL	NULL	VCP	GP		bind					Thio-ataxin-3Q20	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6469_s_379	12944474	(B) Binding of VCP by Thio-ataxin-3Q20.	bind
12166	1	3700	7	11	NULL	NULL	NULL	VCP	GP		bind					Thio-ataxin-3Q20	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6469_s_379	12944474	(B) Binding of VCP by Thio-ataxin-3Q20.	bind
81363	1	3700	11	NULL	NULL	0	NULL	VCP	GeneOrProtein		binds to 					Thio-ataxin-3Q20	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_18_6469_s_379	12944474	(B) Binding of VCP by Thio-ataxin-3Q20.	bind
8530	1	3701	5	11	NULL	NULL	NULL	Yrb1	GP		bind					Gsp	GP		G12V		NULL		NULL	NULL	NULL	NULL	gw60_genetics_157_3_1089_s_214	11238397	(B) Binding of Yrb1 to Gsp(G12V) was assessed by copurification.	bind
8771	1	3701	6	11	NULL	NULL	NULL	Yrb1	GP		bind					Gsp	GP		G12V		NULL		NULL	NULL	NULL	NULL	gw60_genetics_157_3_1089_s_214	11238397	(B) Binding of Yrb1 to Gsp(G12V) was assessed by copurification.	bind
81364	1	3701	11	NULL	NULL	0	NULL	Yrb1	GeneOrProtein		binds to 					Gsp	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_genetics_157_3_1089_s_214	11238397	(B) Binding of Yrb1 to Gsp(G12V) was assessed by copurification.	bind
8532	1	3702	5	11	NULL	NULL	NULL	NAC	GP		bind					CSF proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_44_1_105_s_68	9030704	(B) Binding of []NAC to CSF proteins.	bind
8772	1	3702	6	11	NULL	NULL	NULL	NAC	GP		bind					CSF proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_44_1_105_s_68	9030704	(B) Binding of []NAC to CSF proteins.	bind
81365	1	3702	11	NULL	NULL	0	NULL	NAC	GeneOrProtein		binds to 					CSF protein	Protein				NULL		0	NULL	NULL	NULL	gw60_brainresmolbrainres_44_1_105_s_68	9030704	(B) Binding of []NAC to CSF proteins.	bind
81367	1	3704	11	NULL	NULL	0	NULL	WAF1 gene	Gene		has binding site for					p53 	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_1_12_s_194	9858527	(B) Binding to the p53 binding site of the  WAF1 gene.	bind
8537	1	3705	5	11	NULL	NULL	NULL	TAK/P-TEFb complex	GP		contain					CDK9	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_209	9491887	(B) Biochemical view of the interaction of Tat with the cyclin T  subunit of the CDK9-containing TAK/P-TEFb complex, and the subsequent cooperative binding of Tat  and TAKPPTEFb to TAR RNA.	bind
8538	2	3705	5	11	NULL	NULL	NULL	cyclin T subunit	GP		is present in					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_209	9491887	(B) Biochemical view of the interaction of Tat with the cyclin T  subunit of the CDK9-containing TAK/P-TEFb complex, and the subsequent cooperative binding of Tat  and TAKPPTEFb to TAR RNA.	bind
8539	3	3705	5	11	NULL	NULL	NULL	Tat	GP		interact with					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_209	9491887	(B) Biochemical view of the interaction of Tat with the cyclin T  subunit of the CDK9-containing TAK/P-TEFb complex, and the subsequent cooperative binding of Tat  and TAKPPTEFb to TAR RNA.	bind
8541	4	3705	5	11	NULL	NULL	NULL	Tat	GP		bind					TAR RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_209	9491887	(B) Biochemical view of the interaction of Tat with the cyclin T  subunit of the CDK9-containing TAK/P-TEFb complex, and the subsequent cooperative binding of Tat  and TAKPPTEFb to TAR RNA.	bind
8542	5	3705	5	11	NULL	NULL	NULL	TAKPPTEFb	GP		bind					TAR RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_209	9491887	(B) Biochemical view of the interaction of Tat with the cyclin T  subunit of the CDK9-containing TAK/P-TEFb complex, and the subsequent cooperative binding of Tat  and TAKPPTEFb to TAR RNA.	bind
8544	6	3705	5	11	NULL	NULL	NULL	statement 4	Process		occurs in cooperation with					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_209	9491887	(B) Biochemical view of the interaction of Tat with the cyclin T  subunit of the CDK9-containing TAK/P-TEFb complex, and the subsequent cooperative binding of Tat  and TAKPPTEFb to TAR RNA.	bind
8545	7	3705	5	11	NULL	NULL	NULL	statement 6	Process		occurs after					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_209	9491887	(B) Biochemical view of the interaction of Tat with the cyclin T  subunit of the CDK9-containing TAK/P-TEFb complex, and the subsequent cooperative binding of Tat  and TAKPPTEFb to TAR RNA.	bind
8773	2	3705	6	11	NULL	NULL	NULL	Tat	GP		interacts with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_209	9491887	(B) Biochemical view of the interaction of Tat with the cyclin T  subunit of the CDK9-containing TAK/P-TEFb complex, and the subsequent cooperative binding of Tat  and TAKPPTEFb to TAR RNA.	bind
8774	3	3705	6	11	NULL	NULL	NULL	Tat	GP		bind					TAR RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_209	9491887	(B) Biochemical view of the interaction of Tat with the cyclin T  subunit of the CDK9-containing TAK/P-TEFb complex, and the subsequent cooperative binding of Tat  and TAKPPTEFb to TAR RNA.	bind
8775	4	3705	6	11	NULL	NULL	NULL	TAKPPTEFb	GP		bind					TAR RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_209	9491887	(B) Biochemical view of the interaction of Tat with the cyclin T  subunit of the CDK9-containing TAK/P-TEFb complex, and the subsequent cooperative binding of Tat  and TAKPPTEFb to TAR RNA.	bind
8776	5	3705	6	11	NULL	NULL	NULL	statement 3	Process		acts in cooperation with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_209	9491887	(B) Biochemical view of the interaction of Tat with the cyclin T  subunit of the CDK9-containing TAK/P-TEFb complex, and the subsequent cooperative binding of Tat  and TAKPPTEFb to TAR RNA.	bind
53452	1	3705	6	11	NULL	NULL	NULL	TAK/P-TEFb complex	GP		contain					CDK9	GP		cyclin T subunit		NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_209	9491887	(B) Biochemical view of the interaction of Tat with the cyclin T  subunit of the CDK9-containing TAK/P-TEFb complex, and the subsequent cooperative binding of Tat  and TAKPPTEFb to TAR RNA.	bind
53457	6	3705	6	11	NULL	NULL	NULL	statement 5	Process		occurs after					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_209	9491887	(B) Biochemical view of the interaction of Tat with the cyclin T  subunit of the CDK9-containing TAK/P-TEFb complex, and the subsequent cooperative binding of Tat  and TAKPPTEFb to TAR RNA.	bind
81368	1	3705	11	NULL	NULL	0	NULL	Tat	GeneOrProtein		interact with					cyclin T	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_cell_92_4_451_s_209	9491887	(B) Biochemical view of the interaction of Tat with the cyclin T  subunit of the CDK9-containing TAK/P-TEFb complex, and the subsequent cooperative binding of Tat  and TAKPPTEFb to TAR RNA.	bind
81370	2	3705	11	NULL	NULL	0	NULL	TAK/P-TEFb complex	Protein		contain					CDK9	Protein				NULL		0	NULL	NULL	NULL	gw60_cell_92_4_451_s_209	9491887	(B) Biochemical view of the interaction of Tat with the cyclin T  subunit of the CDK9-containing TAK/P-TEFb complex, and the subsequent cooperative binding of Tat  and TAKPPTEFb to TAR RNA.	bind
81371	3	3705	11	NULL	NULL	0	NULL	cyclin T	Protein		is a subunit of					statement 2	Protein				NULL		0	NULL	NULL	NULL	gw60_cell_92_4_451_s_209	9491887	(B) Biochemical view of the interaction of Tat with the cyclin T  subunit of the CDK9-containing TAK/P-TEFb complex, and the subsequent cooperative binding of Tat  and TAKPPTEFb to TAR RNA.	bind
81372	4	3705	11	NULL	NULL	0	NULL	Tat	GeneOrProtein		binds to 					TAR 	NucleicAcidSubstance	RNA			NULL		0	NULL	NULL	NULL	gw60_cell_92_4_451_s_209	9491887	(B) Biochemical view of the interaction of Tat with the cyclin T  subunit of the CDK9-containing TAK/P-TEFb complex, and the subsequent cooperative binding of Tat  and TAKPPTEFb to TAR RNA.	bind
81373	5	3705	11	NULL	NULL	0	NULL	TAKPPTEFb	Protein		binds to 					TAR	NucleicAcidSubstance	RNA			NULL		0	NULL	NULL	NULL	gw60_cell_92_4_451_s_209	9491887	(B) Biochemical view of the interaction of Tat with the cyclin T  subunit of the CDK9-containing TAK/P-TEFb complex, and the subsequent cooperative binding of Tat  and TAKPPTEFb to TAR RNA.	bind
8553	1	3706	5	11	NULL	NULL	NULL	dopamine	Chemical		stimulate					GTP S	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_brainres_920_1_41_s_181	11716810	(B) Blockade of dopamine (1 mM)-stimulated [35]GTP S binding by the D2/D3 receptor antagonists, raclopride and L741,626.	bind
8554	2	3706	5	11	NULL	NULL	NULL	raclopride	Chemical		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_brainres_920_1_41_s_181	11716810	(B) Blockade of dopamine (1 mM)-stimulated [35]GTP S binding by the D2/D3 receptor antagonists, raclopride and L741,626.	bind
8555	3	3706	5	11	NULL	NULL	NULL	L741,626	Chemical		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_brainres_920_1_41_s_181	11716810	(B) Blockade of dopamine (1 mM)-stimulated [35]GTP S binding by the D2/D3 receptor antagonists, raclopride and L741,626.	bind
44772	4	3706	5	11	NULL	NULL	NULL	raclopride \t	Chemical		is a type of					D2/D3 receptor antagonist	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_brainres_920_1_41_s_181	11716810	(B) Blockade of dopamine (1 mM)-stimulated [35]GTP S binding by the D2/D3 receptor antagonists, raclopride and L741,626.	bind
44773	5	3706	5	11	NULL	NULL	NULL	L741,626	Chemical		is a type of					D2/D3 receptor antagonist	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_brainres_920_1_41_s_181	11716810	(B) Blockade of dopamine (1 mM)-stimulated [35]GTP S binding by the D2/D3 receptor antagonists, raclopride and L741,626.	bind
8777	1	3706	6	11	NULL	NULL	NULL	dopamine	Chemical		stimulates					GTP S	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_brainres_920_1_41_s_181	11716810	(B) Blockade of dopamine (1 mM)-stimulated [35]GTP S binding by the D2/D3 receptor antagonists, raclopride and L741,626.	bind
8778	2	3706	6	11	NULL	NULL	NULL	raclopride	Chemical		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_brainres_920_1_41_s_181	11716810	(B) Blockade of dopamine (1 mM)-stimulated [35]GTP S binding by the D2/D3 receptor antagonists, raclopride and L741,626.	bind
8779	3	3706	6	11	NULL	NULL	NULL	L741,626	Chemical		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_brainres_920_1_41_s_181	11716810	(B) Blockade of dopamine (1 mM)-stimulated [35]GTP S binding by the D2/D3 receptor antagonists, raclopride and L741,626.	bind
40947	4	3706	6	11	NULL	NULL	NULL	raclopride	Chemical		is a type of					D2/D3 receptor antagonist	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_brainres_920_1_41_s_181	11716810	(B) Blockade of dopamine (1 mM)-stimulated [35]GTP S binding by the D2/D3 receptor antagonists, raclopride and L741,626.	bind
40948	5	3706	6	11	NULL	NULL	NULL	L741,626	Chemical		is a type of					D2/D3 receptor antagonist	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_brainres_920_1_41_s_181	11716810	(B) Blockade of dopamine (1 mM)-stimulated [35]GTP S binding by the D2/D3 receptor antagonists, raclopride and L741,626.	bind
81375	1	3706	11	NULL	NULL	0	NULL	raclopride	NonProteinOrNucleicAcidChemical		is an agonist of					D2/D3 receptor 	Protein				NULL		0	NULL	NULL	NULL	gw60_brainres_920_1_41_s_181	11716810	(B) Blockade of dopamine (1 mM)-stimulated [35]GTP S binding by the D2/D3 receptor antagonists, raclopride and L741,626.	bind
81376	2	3706	11	NULL	NULL	0	NULL	L741,626	NonProteinOrNucleicAcidChemical		is an agonist of					D2/D3 receptor 	Protein				NULL		0	NULL	NULL	NULL	gw60_brainres_920_1_41_s_181	11716810	(B) Blockade of dopamine (1 mM)-stimulated [35]GTP S binding by the D2/D3 receptor antagonists, raclopride and L741,626.	bind
81377	3	3706	11	NULL	NULL	0	NULL	dopamine	NonProteinOrNucleicAcidChemical		stimulate					GTP	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	gw60_brainres_920_1_41_s_181	11716810	(B) Blockade of dopamine (1 mM)-stimulated [35]GTP S binding by the D2/D3 receptor antagonists, raclopride and L741,626.	bind
81379	4	3706	11	NULL	NULL	0	NULL	raclopride	NonProteinOrNucleicAcidChemical		blocks					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_brainres_920_1_41_s_181	11716810	(B) Blockade of dopamine (1 mM)-stimulated [35]GTP S binding by the D2/D3 receptor antagonists, raclopride and L741,626.	bind
81380	5	3706	11	NULL	NULL	0	NULL	L741,626	NonProteinOrNucleicAcidChemical		blocks					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_brainres_920_1_41_s_181	11716810	(B) Blockade of dopamine (1 mM)-stimulated [35]GTP S binding by the D2/D3 receptor antagonists, raclopride and L741,626.	bind
8556	1	3707	5	11	NULL	NULL	NULL	UL18-Fc	GP		bind					NK cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_immunity_7_2_273_s_121	9285411	(B) Blocking of binding of UL18-Fc to NK cells by anti-LIR-1.	bind
8557	2	3707	5	11	NULL	NULL	NULL	anti-LIR-1	GP		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_7_2_273_s_121	9285411	(B) Blocking of binding of UL18-Fc to NK cells by anti-LIR-1.	bind
8780	1	3707	6	11	NULL	NULL	NULL	UL18-Fc	GP		bind					NK cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_immunity_7_2_273_s_121	9285411	(B) Blocking of binding of UL18-Fc to NK cells by anti-LIR-1.	bind
8781	2	3707	6	11	NULL	NULL	NULL	anti-LIR-1	GP		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_7_2_273_s_121	9285411	(B) Blocking of binding of UL18-Fc to NK cells by anti-LIR-1.	bind
81382	1	3707	11	NULL	NULL	0	NULL	UL18-Fc	GeneOrProtein		binds to 					NK cells	Cell				NULL		0	NULL	NULL	NULL	gw60_immunity_7_2_273_s_121	9285411	(B) Blocking of binding of UL18-Fc to NK cells by anti-LIR-1.	bind
81383	2	3707	11	NULL	NULL	0	NULL	anti-LIR-1	GeneOrProtein		blocks					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_immunity_7_2_273_s_121	9285411	(B) Blocking of binding of UL18-Fc to NK cells by anti-LIR-1.	bind
8582	1	3708	5	11	NULL	NULL	NULL	Rac1	GP		bind					GST-PAK	GP		GBD		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_125	10508610	(b) Both PAK and N-WASP CRIB peptides inhibit binding of Rac1 and Cdc42 to GST-PAK GBD.	bind
8583	2	3708	5	11	NULL	NULL	NULL	Cdc42	GP		bind					GST-PAK	GP		GBD		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_125	10508610	(b) Both PAK and N-WASP CRIB peptides inhibit binding of Rac1 and Cdc42 to GST-PAK GBD.	bind
8584	3	3708	5	11	NULL	NULL	NULL	PAK	GP		inhibit			CRIB peptide		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_125	10508610	(b) Both PAK and N-WASP CRIB peptides inhibit binding of Rac1 and Cdc42 to GST-PAK GBD.	bind
8586	4	3708	5	11	NULL	NULL	NULL	PAK	GP		inhibit			CRIB peptide		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_125	10508610	(b) Both PAK and N-WASP CRIB peptides inhibit binding of Rac1 and Cdc42 to GST-PAK GBD.	bind
8587	5	3708	5	11	NULL	NULL	NULL	N-WASP	GP		inhibit			CRIB peptide		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_125	10508610	(b) Both PAK and N-WASP CRIB peptides inhibit binding of Rac1 and Cdc42 to GST-PAK GBD.	bind
8588	6	3708	5	11	NULL	NULL	NULL	N-WASP	GP		inhibit			CRIB peptide		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_125	10508610	(b) Both PAK and N-WASP CRIB peptides inhibit binding of Rac1 and Cdc42 to GST-PAK GBD.	bind
8782	1	3708	6	11	NULL	NULL	NULL	Rac1	GP		bind					GST-PAK	GP		GBD		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_125	10508610	(b) Both PAK and N-WASP CRIB peptides inhibit binding of Rac1 and Cdc42 to GST-PAK GBD.	bind
8783	2	3708	6	11	NULL	NULL	NULL	Cdc42	GP		bind					GST-PAK	GP		GBD		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_125	10508610	(b) Both PAK and N-WASP CRIB peptides inhibit binding of Rac1 and Cdc42 to GST-PAK GBD.	bind
8784	3	3708	6	11	NULL	NULL	NULL	PAK	GP		inhibits			 CRIB peptide		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_125	10508610	(b) Both PAK and N-WASP CRIB peptides inhibit binding of Rac1 and Cdc42 to GST-PAK GBD.	bind
8785	4	3708	6	11	NULL	NULL	NULL	PAK	GP		inhibits			CRIB peptide		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_125	10508610	(b) Both PAK and N-WASP CRIB peptides inhibit binding of Rac1 and Cdc42 to GST-PAK GBD.	bind
8786	5	3708	6	11	NULL	NULL	NULL	N-WASP	GP		inhibits			 CRIB peptide		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_125	10508610	(b) Both PAK and N-WASP CRIB peptides inhibit binding of Rac1 and Cdc42 to GST-PAK GBD.	bind
8787	6	3708	6	11	NULL	NULL	NULL	N-WASP	GP		inhibits			 CRIB peptide		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_125	10508610	(b) Both PAK and N-WASP CRIB peptides inhibit binding of Rac1 and Cdc42 to GST-PAK GBD.	bind
81384	1	3708	11	NULL	NULL	0	NULL	Rac1	GeneOrProtein		binds to 					GST-PAK GBD	Protein				NULL		0	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_125	10508610	(b) Both PAK and N-WASP CRIB peptides inhibit binding of Rac1 and Cdc42 to GST-PAK GBD.	bind
81385	2	3708	11	NULL	NULL	0	NULL	Cdc42	GeneOrProtein		binds to 					GST-PAK GBD	Protein				NULL		0	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_125	10508610	(b) Both PAK and N-WASP CRIB peptides inhibit binding of Rac1 and Cdc42 to GST-PAK GBD.	bind
81386	3	3708	11	NULL	NULL	0	NULL	PAK	PartOfProtein	peptide	inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_125	10508610	(b) Both PAK and N-WASP CRIB peptides inhibit binding of Rac1 and Cdc42 to GST-PAK GBD.	bind
81387	4	3708	11	NULL	NULL	0	NULL	PAK	PartOfProtein	peptide	inhibit					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_125	10508610	(b) Both PAK and N-WASP CRIB peptides inhibit binding of Rac1 and Cdc42 to GST-PAK GBD.	bind
81388	5	3708	11	NULL	NULL	0	NULL	N-WASP CRIB	PartOfProtein	peptide	inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_125	10508610	(b) Both PAK and N-WASP CRIB peptides inhibit binding of Rac1 and Cdc42 to GST-PAK GBD.	bind
81389	6	3708	11	NULL	NULL	0	NULL	N-WASP CRIB	PartOfProtein	peptide	inhibit					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_currbiol_9_18_991_s_125	10508610	(b) Both PAK and N-WASP CRIB peptides inhibit binding of Rac1 and Cdc42 to GST-PAK GBD.	bind
8589	1	3709	5	11	NULL	NULL	NULL	Vg1RBP/Vera	GP		bind		specifically			Xcat2	GP			 3'UTR	NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_10_4669_s_239	15292452	(B) Both Vg1RBP/Vera and VgRBP60/hnRNP I specifically bind to the Xcat2  3'UTR.	bind
8590	2	3709	5	11	NULL	NULL	NULL	VgRBP60/hnRNP I	GP		bind		specifically			Xcat2	GP			3'UTR	NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_10_4669_s_239	15292452	(B) Both Vg1RBP/Vera and VgRBP60/hnRNP I specifically bind to the Xcat2  3'UTR.	bind
8788	1	3709	6	11	NULL	NULL	NULL	Vg1RBP/Vera	GP		bind		specifically			Xcat2 	GP			3'UTR	NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_10_4669_s_239	15292452	(B) Both Vg1RBP/Vera and VgRBP60/hnRNP I specifically bind to the Xcat2  3'UTR.	bind
8789	2	3709	6	11	NULL	NULL	NULL	VgRBP60/hnRNP I	GP		bind		specifically			Xcat2 	GP			3'UTR	NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_10_4669_s_239	15292452	(B) Both Vg1RBP/Vera and VgRBP60/hnRNP I specifically bind to the Xcat2  3'UTR.	bind
81390	1	3709	11	NULL	NULL	0	NULL	Vg1RBP/Vera	GeneOrProtein		binds to 		specifically			Xcat2 	Gene			3'UTR	NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_10_4669_s_239	15292452	(B) Both Vg1RBP/Vera and VgRBP60/hnRNP I specifically bind to the Xcat2  3'UTR.	bind
81391	2	3709	11	NULL	NULL	0	NULL	VgRBP60/hnRNP I	GeneOrProtein		binds to 					Xcat2 	Gene			3'UTR	NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_10_4669_s_239	15292452	(B) Both Vg1RBP/Vera and VgRBP60/hnRNP I specifically bind to the Xcat2  3'UTR.	bind
8591	1	3711	5	11	NULL	NULL	NULL	BRG1	GP		bind					p21	GP	endogenous		promoter	NULL	HeLa cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_3_1188_s_96	14729964	(B) BRG1 is bound to the endogenous p21 promoter (p21 pr) in HeLa cells.	bind
10035	2	3711	5	11	NULL	NULL	NULL	p21 pr	GP		is					promoter p21	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_3_1188_s_96	14729964	(B) BRG1 is bound to the endogenous p21 promoter (p21 pr) in HeLa cells.	bind
8790	1	3711	6	11	NULL	NULL	NULL	BRG1	GP		bind					p21	GP	endogenous		promoter	NULL	HeLa cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_3_1188_s_96	14729964	(B) BRG1 is bound to the endogenous p21 promoter (p21 pr) in HeLa cells.	bind
8791	2	3711	6	11	NULL	NULL	NULL	p21 pr	GP		is					p21 promoter	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_3_1188_s_96	14729964	(B) BRG1 is bound to the endogenous p21 promoter (p21 pr) in HeLa cells.	bind
81392	1	3711	11	NULL	NULL	0	NULL	BRG1	GeneOrProtein		binds to 					p21	Gene	endogenous		promoter	NULL	HeLa cell	0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1188_s_96	14729964	(B) BRG1 is bound to the endogenous p21 promoter (p21 pr) in HeLa cells.	bind
8592	1	3712	5	11	NULL	NULL	NULL	c-IAP1	GP		bind					c-IAP2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3348_s_242	15798218	(B) c-IAP1 binds c-IAP2 only in the presence of TRAF1 or TRAF2.	bind
8593	2	3712	5	11	NULL	NULL	NULL	statement 1	Process		in the presence of		only			TRAF1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3348_s_242	15798218	(B) c-IAP1 binds c-IAP2 only in the presence of TRAF1 or TRAF2.	bind
8594	3	3712	5	11	NULL	NULL	NULL	statement 1	Process		in the presence of		only			TRAF2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3348_s_242	15798218	(B) c-IAP1 binds c-IAP2 only in the presence of TRAF1 or TRAF2.	bind
8596	4	3712	5	11	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3348_s_242	15798218	(B) c-IAP1 binds c-IAP2 only in the presence of TRAF1 or TRAF2.	bind
8793	1	3712	6	11	NULL	NULL	NULL	c-IAP1	GP		bind					c-IAP2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3348_s_242	15798218	(B) c-IAP1 binds c-IAP2 only in the presence of TRAF1 or TRAF2.	bind
8794	2	3712	6	11	NULL	NULL	NULL	statement 1	Process		occurs in presence of		only			TRAF1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3348_s_242	15798218	(B) c-IAP1 binds c-IAP2 only in the presence of TRAF1 or TRAF2.	bind
8795	3	3712	6	11	NULL	NULL	NULL	statement 1	Process		occurs in presence of		only			TRAF2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3348_s_242	15798218	(B) c-IAP1 binds c-IAP2 only in the presence of TRAF1 or TRAF2.	bind
8796	4	3712	6	11	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3348_s_242	15798218	(B) c-IAP1 binds c-IAP2 only in the presence of TRAF1 or TRAF2.	bind
81393	1	3712	11	NULL	NULL	0	NULL	c-IAP1	GeneOrProtein		binds to 					c-IAP2 	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_8_3348_s_242	15798218	(B) c-IAP1 binds c-IAP2 only in the presence of TRAF1 or TRAF2.	bind
81394	2	3712	11	NULL	NULL	0	NULL	statement 1	Process		occurs in the presence of					TRAF1	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_8_3348_s_242	15798218	(B) c-IAP1 binds c-IAP2 only in the presence of TRAF1 or TRAF2.	bind
81395	3	3712	11	NULL	NULL	0	NULL	statement 1	Process		occurs in the presence of					TRAF2	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_8_3348_s_242	15798218	(B) c-IAP1 binds c-IAP2 only in the presence of TRAF1 or TRAF2.	bind
8597	1	3713	5	11	NULL	NULL	NULL	Sso	GP		bind					Vsm1	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molbiolcell_14_8_3114_s_193	12925750	(B) C2-ceramide inhibits the binding of Sso to Vsm1 in vivo.	bind
8598	2	3713	5	11	NULL	NULL	NULL	C2-ceramide	Chemical		inhibit					statement 1	Process				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molbiolcell_14_8_3114_s_193	12925750	(B) C2-ceramide inhibits the binding of Sso to Vsm1 in vivo.	bind
8797	1	3713	6	11	NULL	NULL	NULL	Sso	GP		bind					Vsm1	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molbiolcell_14_8_3114_s_193	12925750	(B) C2-ceramide inhibits the binding of Sso to Vsm1 in vivo.	bind
8798	2	3713	6	11	NULL	NULL	NULL	C2-ceramide	Chemical		inhibits					statement 1	Process				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molbiolcell_14_8_3114_s_193	12925750	(B) C2-ceramide inhibits the binding of Sso to Vsm1 in vivo.	bind
81396	1	3713	11	NULL	NULL	0	NULL	C2-ceramide	Chemical		inhibit					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_8_3114_s_193	12925750	(B) C2-ceramide inhibits the binding of Sso to Vsm1 in vivo.	bind
81397	2	3713	11	NULL	NULL	0	NULL	Sso	GeneOrProtein		binds to 					Vsm1	GeneOrProtein				NULL	in vivo	0	NULL	NULL	NULL	gw60_molbiolcell_14_8_3114_s_193	12925750	(B) C2-ceramide inhibits the binding of Sso to Vsm1 in vivo.	bind
8600	1	3714	5	11	NULL	NULL	NULL	brain proteins	GP		bind					syntaxin-1A	GP		191-240		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_155	16030255	(B) Ca2+-dependent binding of brain proteins to syntaxin-1A [191-240] and syntaxin-1A [191-240  L222].	bind
8601	2	3714	5	11	NULL	NULL	NULL	statement 1	Process		is dependent on					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_155	16030255	(B) Ca2+-dependent binding of brain proteins to syntaxin-1A [191-240] and syntaxin-1A [191-240  L222].	bind
8603	3	3714	5	11	NULL	NULL	NULL	brain proteins	GP		bind					syntaxin-1A	GP		191-240;; L222		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_155	16030255	(B) Ca2+-dependent binding of brain proteins to syntaxin-1A [191-240] and syntaxin-1A [191-240  L222].	bind
8604	4	3714	5	11	NULL	NULL	NULL	statement 3	Process		is dependent on					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_155	16030255	(B) Ca2+-dependent binding of brain proteins to syntaxin-1A [191-240] and syntaxin-1A [191-240  L222].	bind
8799	1	3714	6	11	NULL	NULL	NULL	brain proteins	GP		bind					syntaxin-1A	GP		191-240		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_155	16030255	(B) Ca2+-dependent binding of brain proteins to syntaxin-1A [191-240] and syntaxin-1A [191-240  L222].	bind
8800	2	3714	6	11	NULL	NULL	NULL	brain proteins	GP		bind					syntaxin-1A	GP		191-240;;L222		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_155	16030255	(B) Ca2+-dependent binding of brain proteins to syntaxin-1A [191-240] and syntaxin-1A [191-240  L222].	bind
8801	3	3714	6	11	NULL	NULL	NULL	statement 1	Process		is dependent on					Ca+2	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_155	16030255	(B) Ca2+-dependent binding of brain proteins to syntaxin-1A [191-240] and syntaxin-1A [191-240  L222].	bind
8802	4	3714	6	11	NULL	NULL	NULL	statement 2	Process		is dependent on					Ca+2	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_155	16030255	(B) Ca2+-dependent binding of brain proteins to syntaxin-1A [191-240] and syntaxin-1A [191-240  L222].	bind
81398	1	3714	11	NULL	NULL	0	NULL	brain proteins	Protein		binds to 					syntaxin-1A	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_155	16030255	(B) Ca2+-dependent binding of brain proteins to syntaxin-1A [191-240] and syntaxin-1A [191-240  L222].	bind
81399	2	3714	11	NULL	NULL	0	NULL	brain proteins	Protein		binds to 					syntaxin-1A	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_155	16030255	(B) Ca2+-dependent binding of brain proteins to syntaxin-1A [191-240] and syntaxin-1A [191-240  L222].	bind
81400	3	3714	11	NULL	NULL	0	NULL	statement 1	Process		depends on					Ca2+	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_155	16030255	(B) Ca2+-dependent binding of brain proteins to syntaxin-1A [191-240] and syntaxin-1A [191-240  L222].	bind
81401	4	3714	11	NULL	NULL	0	NULL	statement 2	Process		depends on					Ca2+	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_155	16030255	(B) Ca2+-dependent binding of brain proteins to syntaxin-1A [191-240] and syntaxin-1A [191-240  L222].	bind
8606	1	3718	5	11	NULL	NULL	NULL	CAT	GP		bind					SHP2	GP				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_91	15556604	(B) CAT binds SHP2 upon stimulation with FBS or laminin  (LA), but not with hyaluronic acid (HA) or elastin (EL).	bind
8608	2	3718	5	11	NULL	NULL	NULL	FBS	CellComponent		stimulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_91	15556604	(B) CAT binds SHP2 upon stimulation with FBS or laminin  (LA), but not with hyaluronic acid (HA) or elastin (EL).	bind
8609	3	3718	5	11	NULL	NULL	NULL	LA	GP		stimulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_91	15556604	(B) CAT binds SHP2 upon stimulation with FBS or laminin  (LA), but not with hyaluronic acid (HA) or elastin (EL).	bind
8610	4	3718	5	11	NULL	NULL	NULL	LA	GP		is					laminin	GP				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_91	15556604	(B) CAT binds SHP2 upon stimulation with FBS or laminin  (LA), but not with hyaluronic acid (HA) or elastin (EL).	bind
8612	5	3718	5	11	NULL	NULL	NULL	HA	Chemical		does not stimulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_91	15556604	(B) CAT binds SHP2 upon stimulation with FBS or laminin  (LA), but not with hyaluronic acid (HA) or elastin (EL).	bind
8613	6	3718	5	11	NULL	NULL	NULL	HA	Chemical		is					hyaluronic acid	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_91	15556604	(B) CAT binds SHP2 upon stimulation with FBS or laminin  (LA), but not with hyaluronic acid (HA) or elastin (EL).	bind
8614	7	3718	5	11	NULL	NULL	NULL	EL	GP		does not stimulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_91	15556604	(B) CAT binds SHP2 upon stimulation with FBS or laminin  (LA), but not with hyaluronic acid (HA) or elastin (EL).	bind
8615	8	3718	5	11	NULL	NULL	NULL	EL	GP		is					elastin	GP				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_91	15556604	(B) CAT binds SHP2 upon stimulation with FBS or laminin  (LA), but not with hyaluronic acid (HA) or elastin (EL).	bind
8803	1	3718	6	11	NULL	NULL	NULL	CAT	GP		bind					SHP2	GP				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_91	15556604	(B) CAT binds SHP2 upon stimulation with FBS or laminin  (LA), but not with hyaluronic acid (HA) or elastin (EL).	bind
8804	2	3718	6	11	NULL	NULL	NULL	FBS	CellComponent		stimulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_91	15556604	(B) CAT binds SHP2 upon stimulation with FBS or laminin  (LA), but not with hyaluronic acid (HA) or elastin (EL).	bind
8805	3	3718	6	11	NULL	NULL	NULL	LA	GP		stimulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_91	15556604	(B) CAT binds SHP2 upon stimulation with FBS or laminin  (LA), but not with hyaluronic acid (HA) or elastin (EL).	bind
8806	4	3718	6	11	NULL	NULL	NULL	LA	GP		is					laminin	GP				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_91	15556604	(B) CAT binds SHP2 upon stimulation with FBS or laminin  (LA), but not with hyaluronic acid (HA) or elastin (EL).	bind
8807	5	3718	6	11	NULL	NULL	NULL	HA	Chemical		does not stimulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_91	15556604	(B) CAT binds SHP2 upon stimulation with FBS or laminin  (LA), but not with hyaluronic acid (HA) or elastin (EL).	bind
8808	6	3718	6	11	NULL	NULL	NULL	EL	GP		does not stimulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_91	15556604	(B) CAT binds SHP2 upon stimulation with FBS or laminin  (LA), but not with hyaluronic acid (HA) or elastin (EL).	bind
8809	7	3718	6	11	NULL	NULL	NULL	HA	Chemical		is					hyaluronic acid	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_91	15556604	(B) CAT binds SHP2 upon stimulation with FBS or laminin  (LA), but not with hyaluronic acid (HA) or elastin (EL).	bind
8810	8	3718	6	11	NULL	NULL	NULL	EL 	GP		is					elastin	GP				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_91	15556604	(B) CAT binds SHP2 upon stimulation with FBS or laminin  (LA), but not with hyaluronic acid (HA) or elastin (EL).	bind
8811	9	3718	6	11	NULL	NULL	NULL	statement 5	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_91	15556604	(B) CAT binds SHP2 upon stimulation with FBS or laminin  (LA), but not with hyaluronic acid (HA) or elastin (EL).	bind
81402	1	3718	11	NULL	NULL	0	NULL	CAT	GeneOrProtein		binds to 					SHP2	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw70_febslett_577_3_327_s_91	15556604	(B) CAT binds SHP2 upon stimulation with FBS or laminin  (LA), but not with hyaluronic acid (HA) or elastin (EL).	bind
81403	2	3718	11	NULL	NULL	0	NULL	FBS	Chemical		stimulates					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_febslett_577_3_327_s_91	15556604	(B) CAT binds SHP2 upon stimulation with FBS or laminin  (LA), but not with hyaluronic acid (HA) or elastin (EL).	bind
81404	3	3718	11	NULL	NULL	0	NULL	laminin	GeneOrProtein		stimulates					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_febslett_577_3_327_s_91	15556604	(B) CAT binds SHP2 upon stimulation with FBS or laminin  (LA), but not with hyaluronic acid (HA) or elastin (EL).	bind
81405	4	3718	11	NULL	NULL	0	NULL	laminin	GeneOrProtein		is					LA	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw70_febslett_577_3_327_s_91	15556604	(B) CAT binds SHP2 upon stimulation with FBS or laminin  (LA), but not with hyaluronic acid (HA) or elastin (EL).	bind
81406	5	3718	11	NULL	NULL	0	NULL	hyaluronic acid	NonProteinOrNucleicAcidChemical		is					HA	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	gw70_febslett_577_3_327_s_91	15556604	(B) CAT binds SHP2 upon stimulation with FBS or laminin  (LA), but not with hyaluronic acid (HA) or elastin (EL).	bind
81407	6	3718	11	NULL	NULL	NULL	NULL	EL	GeneOrProtein		is					elastin	GeneOrProtein				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_91	15556604	(B) CAT binds SHP2 upon stimulation with FBS or laminin  (LA), but not with hyaluronic acid (HA) or elastin (EL).	bind
81408	7	3718	11	NULL	NULL	0	NULL	hyaluronic acid	NonProteinOrNucleicAcidChemical		does not stimulate					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_febslett_577_3_327_s_91	15556604	(B) CAT binds SHP2 upon stimulation with FBS or laminin  (LA), but not with hyaluronic acid (HA) or elastin (EL).	bind
81409	8	3718	11	NULL	NULL	NULL	NULL	elastin	GeneOrProtein		does not stimulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_91	15556604	(B) CAT binds SHP2 upon stimulation with FBS or laminin  (LA), but not with hyaluronic acid (HA) or elastin (EL).	bind
8616	1	3719	5	11	NULL	NULL	NULL	SATB1 DNA	NucleicAcid		bind					MMTV	Organism			LTR	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4918_s_214	10373541	(B) CDP overexpression prevents SATB1 DNA binding to the MMTV LTR.	bind
8617	2	3719	5	11	NULL	NULL	NULL	CDP	GP	overexpression of	prevent					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4918_s_214	10373541	(B) CDP overexpression prevents SATB1 DNA binding to the MMTV LTR.	bind
8812	1	3719	6	11	NULL	NULL	NULL	SATB1 DNA	NucleicAcid		bind					MMTV	Organism			LTR	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4918_s_214	10373541	(B) CDP overexpression prevents SATB1 DNA binding to the MMTV LTR.	bind
8813	2	3719	6	11	NULL	NULL	NULL	CDP	GP	overexpression of	prevents					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4918_s_214	10373541	(B) CDP overexpression prevents SATB1 DNA binding to the MMTV LTR.	bind
81410	1	3719	11	NULL	NULL	NULL	NULL	SATB1	Gene	DNA	binds to 					MMTV	Gene	LTR			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4918_s_214	10373541	(B) CDP overexpression prevents SATB1 DNA binding to the MMTV LTR.	bind
81411	2	3719	11	NULL	NULL	0	NULL	CDP	Gene	overexpression	prevents					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_7_4918_s_214	10373541	(B) CDP overexpression prevents SATB1 DNA binding to the MMTV LTR.	bind
10032	1	3720	5	11	NULL	NULL	NULL	amphiphysin	GP	mutant	does not bind			SH3 domain					proline-rich sequences		NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_45_6_787_s_146	14529717	(B) Cells overexpressing transfected G684R/P687L mutant amphiphysin SH3 domain (which  no longer binds to proline-rich sequences), stained for either the mutant SH3 domain  (left), or for internalized transferrin (Tf, right).	bind
8814	1	3720	6	11	NULL	NULL	NULL	amphiphysin	GP	mutant	does not bind			SH3 domain					proline-rich sequences		NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_45_6_787_s_146	14529717	(B) Cells overexpressing transfected G684R/P687L mutant amphiphysin SH3 domain (which  no longer binds to proline-rich sequences), stained for either the mutant SH3 domain  (left), or for internalized transferrin (Tf, right).	bind
81412	1	3720	11	NULL	NULL	0	NULL	amphiphysin	Protein	 G684R/P687L mutant 	does not bind to			SH3 domain		proline-rich sequence	PartOfProtein				NULL		0	NULL	NULL	NULL	gw70_neuropharmacology_45_6_787_s_146	14529717	(B) Cells overexpressing transfected G684R/P687L mutant amphiphysin SH3 domain (which  no longer binds to proline-rich sequences), stained for either the mutant SH3 domain  (left), or for internalized transferrin (Tf, right).	bind
8623	1	3721	5	11	NULL	NULL	NULL	Ssb1/2p	GP		bind					HSF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_5_1739_s_270	10793148	(B) Cells were grown in 0.5% glucose to induce the binding of Ssb1/2p to HSF.	bind
8624	2	3721	5	11	NULL	NULL	NULL	glucose	Chemical		induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_5_1739_s_270	10793148	(B) Cells were grown in 0.5% glucose to induce the binding of Ssb1/2p to HSF.	bind
8815	1	3721	6	11	NULL	NULL	NULL	Ssb1/2p	GP		bind					HSF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_5_1739_s_270	10793148	(B) Cells were grown in 0.5% glucose to induce the binding of Ssb1/2p to HSF.	bind
8816	2	3721	6	11	NULL	NULL	NULL	glucose	Chemical		induces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_5_1739_s_270	10793148	(B) Cells were grown in 0.5% glucose to induce the binding of Ssb1/2p to HSF.	bind
81413	1	3721	11	NULL	NULL	0	NULL	 Ssb1/2p	Protein		binds to 					HSF	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_5_1739_s_270	10793148	(B) Cells were grown in 0.5% glucose to induce the binding of Ssb1/2p to HSF.	bind
81414	2	3721	11	NULL	NULL	0	NULL	glucose	NonProteinOrNucleicAcidChemical		induces					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_5_1739_s_270	10793148	(B) Cells were grown in 0.5% glucose to induce the binding of Ssb1/2p to HSF.	bind
8625	1	3724	5	11	NULL	NULL	NULL	CREB	GP		bind					NF-IL6beta gene locus	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_7_3365_s_199	15901830	(B) ChIP analysis of CREB or Sp1 binding to  the  NF-IL6beta gene locus.	bind
10030	2	3724	5	11	NULL	NULL	NULL	Sp1	GP		bind					NF-IL6beta gene locus	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_7_3365_s_199	15901830	(B) ChIP analysis of CREB or Sp1 binding to  the  NF-IL6beta gene locus.	bind
10031	3	3724	5	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_7_3365_s_199	15901830	(B) ChIP analysis of CREB or Sp1 binding to  the  NF-IL6beta gene locus.	bind
8817	1	3724	6	11	NULL	NULL	NULL	CREB	GP		bind					NF-IL6beta gene	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_7_3365_s_199	15901830	(B) ChIP analysis of CREB or Sp1 binding to  the  NF-IL6beta gene locus.	bind
8818	2	3724	6	11	NULL	NULL	NULL	Sp1	GP		bind					NF-IL6beta gene	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_7_3365_s_199	15901830	(B) ChIP analysis of CREB or Sp1 binding to  the  NF-IL6beta gene locus.	bind
8819	3	3724	6	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_7_3365_s_199	15901830	(B) ChIP analysis of CREB or Sp1 binding to  the  NF-IL6beta gene locus.	bind
81415	1	3724	11	NULL	NULL	0	NULL	CREB	GeneOrProtein		binds to 					NF-IL6beta gene	Gene			locus	NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_7_3365_s_199	15901830	(B) ChIP analysis of CREB or Sp1 binding to  the  NF-IL6beta gene locus.	bind
81416	2	3724	11	NULL	NULL	0	NULL	Sp1	GeneOrProtein		binds to 					NF-IL6beta gene	Gene			locus	NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_7_3365_s_199	15901830	(B) ChIP analysis of CREB or Sp1 binding to  the  NF-IL6beta gene locus.	bind
8626	1	3725	5	11	NULL	NULL	NULL	PU.1	GP		bind					mcl-1 gene locus	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_6_1896_s_112	12612065	(B) ChIP analysis of PU.1 binding to the  mcl-1 gene locus.	bind
8820	1	3725	6	11	NULL	NULL	NULL	PU.1	GP		bind					mcl-1 gene locus	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_6_1896_s_112	12612065	(B) ChIP analysis of PU.1 binding to the  mcl-1 gene locus.	bind
81417	1	3725	11	NULL	NULL	0	NULL	 PU.1	GeneOrProtein		binds to 					mcl-1 gene	Gene			locus	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_6_1896_s_112	12612065	(B) ChIP analysis of PU.1 binding to the  mcl-1 gene locus.	bind
8627	1	3726	5	11	NULL	NULL	NULL	c-Rel	GP		bind					bfl-1 locus	GP				NULL	in human Jurkat T cells stimulated with PMA plus ionomycin (P+I)	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
8629	2	3726	5	11	NULL	NULL	NULL	p65/RelA	GP		bind					bfl-1 locus	GP				NULL	in human Jurkat T cells stimulated with PMA plus ionomycin (P+I)	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
8630	3	3726	5	11	NULL	NULL	NULL	c-Jun	GP		bind					bfl-1 locus	GP				NULL	in human Jurkat T cells stimulated with PMA plus ionomycin (P+I)	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
8631	4	3726	5	11	NULL	NULL	NULL	C/EBPbeta	GP		bind					bfl-1 locus	GP				NULL	in human Jurkat T cells stimulated with PMA plus ionomycin (P+I)	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
8632	5	3726	5	11	NULL	NULL	NULL	HMGI-C	GP		bind					bfl-1 locus	GP				NULL	in human Jurkat T cells stimulated with PMA plus ionomycin (P+I)	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
8633	6	3726	5	11	NULL	NULL	NULL	c-Rel	GP		bind					bfl-1 locus	GP				NULL	in human Jurkat T cells stimulated with DMSO control	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
8634	7	3726	5	11	NULL	NULL	NULL	p65/RelA	GP		bind					bfl-1 locus	GP				NULL	in human Jurkat T cells stimulated with DMSO control	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
8635	8	3726	5	11	NULL	NULL	NULL	c-Jun	GP		bind					bfl-1 locus	GP				NULL	in human Jurkat T cells stimulated with DMSO control	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
8636	9	3726	5	11	NULL	NULL	NULL	C/EBPbeta	GP		bind					bfl-1 locus	GP				NULL	in human Jurkat T cells stimulated with DMSO control	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
8637	10	3726	5	11	NULL	NULL	NULL	HMGI-C	GP		bind					bfl-1 locus	GP				NULL	in human Jurkat T cells stimulated with DMSO control	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
8638	11	3726	5	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
8639	12	3726	5	11	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
8640	13	3726	5	11	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
8641	14	3726	5	11	NULL	NULL	NULL	statement 4	Process		bind					statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
8642	15	3726	5	11	NULL	NULL	NULL	statement 5	Process		is an alternative to					statement 10	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
53465	16	3726	5	11	NULL	NULL	NULL	c-Rel	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
53466	17	3726	5	11	NULL	NULL	NULL	p65/RelA	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
53467	18	3726	5	11	NULL	NULL	NULL	C/EBPbeta	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
53468	19	3726	5	11	NULL	NULL	NULL	HMGI-C	GP		is a type of					architectural factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
53470	20	3726	5	11	NULL	NULL	NULL	c-Jun	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
8821	1	3726	6	11	NULL	NULL	NULL	c-Rel	GP		bind					bfl-1 locus	GP				NULL	human Jurkat T cells stimulated with PMA plus ionomycin	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
8822	2	3726	6	11	NULL	NULL	NULL	p65/RelA	GP		bind					bfl-1 locus	GP				NULL	human Jurkat T cells stimulated with PMA plus ionomycin	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
8823	3	3726	6	11	NULL	NULL	NULL	c-Jun	GP		bind					bfl-1 locus	GP				NULL	human Jurkat T cells stimulated with PMA plus ionomycin	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
8824	4	3726	6	11	NULL	NULL	NULL	C/EBPbeta	GP		bind					bfl-1 locus	GP				NULL	human Jurkat T cells stimulated with PMA plus ionomycin	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
8825	5	3726	6	11	NULL	NULL	NULL	HMGI-C	GP		bind					bfl-1 locus	GP				NULL	human Jurkat T cells stimulated with PMA plus ionomycin	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
9694	6	3726	6	11	NULL	NULL	NULL	c-Rel	GP		bind					bfl-1 locus	GP				NULL	human Jurkat T cells stimulated with DMSO control	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
9695	7	3726	6	11	NULL	NULL	NULL	p65/RelA	GP		bind					bfl-1 locus	GP				NULL	human Jurkat T cells stimulated with DMSO control	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
9696	8	3726	6	11	NULL	NULL	NULL	c-Jun	GP		bind					bfl-1 locus	GP				NULL	human Jurkat T cells stimulated with DMSO control	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
9697	9	3726	6	11	NULL	NULL	NULL	C/EBPbeta	GP		bind					bfl-1 locus	GP				NULL	human Jurkat T cells stimulated with DMSO control	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
9698	10	3726	6	11	NULL	NULL	NULL	HMGI-C	GP		bind					bfl-1 locus	GP				NULL	human Jurkat T cells stimulated with DMSO control	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
40953	11	3726	6	11	NULL	NULL	NULL	c-Rel	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
40954	12	3726	6	11	NULL	NULL	NULL	p65/RelA	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
40955	13	3726	6	11	NULL	NULL	NULL	c-Jun	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
40956	14	3726	6	11	NULL	NULL	NULL	C/EBPbeta	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
40957	15	3726	6	11	NULL	NULL	NULL	HMGI-C 	GP		is a type of					architectural factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
53469	16	3726	6	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
53471	17	3726	6	11	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
53472	18	3726	6	11	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
53473	19	3726	6	11	NULL	NULL	NULL	statement 4	Process		is an alternative to					statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
53474	20	3726	6	11	NULL	NULL	NULL	statement 5	Process		is an alternative to					statement 10	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
81418	1	3726	11	NULL	NULL	0	NULL	c-Rel	Protein		is a type of 					transcription factor	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
81419	2	3726	11	NULL	NULL	0	NULL	 p65/RelA	Protein		is a type of 					transcription factor	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
81420	3	3726	11	NULL	NULL	0	NULL	c-Jun	Protein		is a type of 					transcription factor	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
81421	4	3726	11	NULL	NULL	0	NULL	C/EBPbeta	Protein		is a type of 					transcription factor	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
81422	5	3726	11	NULL	NULL	0	NULL	HMGI-C	GeneOrProtein		binds to 					bfl-1	Gene	human;;Jurkat T cell		locus	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
81423	6	3726	11	NULL	NULL	0	NULL	PMA 	NonProteinOrNucleicAcidChemical		stimulates					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
81424	7	3726	11	NULL	NULL	0	NULL	 ionomycin	NonProteinOrNucleicAcidChemical		stimulates					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
81425	8	3726	11	NULL	NULL	0	NULL	statement 6	Process		occurs along with					statement 7	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_8_2749_s_222	12665576	(B) ChIP analysis of transcription factors c-Rel, p65/RelA, c-Jun, and  C/EBPbeta and of architectural factor HMGI-C binding to the  bfl-1 locus in human Jurkat T cells stimulated with PMA plus ionomycin (P+I) for 2 or 18  h or with a DMSO control.	bind
8643	1	3727	5	11	NULL	NULL	NULL	Myc	GP		bind					P57KIP2 gene	GP			DNA surrounding the start site of transcription of	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7648_s_228	14560010	(B) ChIp experiments documenting in vivo binding of Myc and Miz1 to DNA surrounding  the start site of transcription of the  P57KIP2and  P21CIP1 genes.	bind
8644	2	3727	5	11	NULL	NULL	NULL	Myc	GP		bind					P21CIP1 gene	GP			DNA surrounding the start site of transcription of	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7648_s_228	14560010	(B) ChIp experiments documenting in vivo binding of Myc and Miz1 to DNA surrounding  the start site of transcription of the  P57KIP2and  P21CIP1 genes.	bind
8645	3	3727	5	11	NULL	NULL	NULL	Miz1	GP		bind					P57KIP2 gene	GP			DNA surrounding the start site of transcription of	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7648_s_228	14560010	(B) ChIp experiments documenting in vivo binding of Myc and Miz1 to DNA surrounding  the start site of transcription of the  P57KIP2and  P21CIP1 genes.	bind
8646	4	3727	5	11	NULL	NULL	NULL	Miz1	GP		bind					P21CIP1 gene	GP			DNA surrounding the start site of transcription of	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7648_s_228	14560010	(B) ChIp experiments documenting in vivo binding of Myc and Miz1 to DNA surrounding  the start site of transcription of the  P57KIP2and  P21CIP1 genes.	bind
8826	1	3727	6	11	NULL	NULL	NULL	Myc	GP		bind					P57KIP2 gene	GP			DNA surrounding transcription start site	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7648_s_228	14560010	(B) ChIp experiments documenting in vivo binding of Myc and Miz1 to DNA surrounding  the start site of transcription of the  P57KIP2and  P21CIP1 genes.	bind
8827	2	3727	6	NULL	NULL	0	NULL	Myc	NULL		bind	NULL				p21Cip1	NULL			DNA surrounding transcription start site	NULL	in vivo	0	NULL	NULL	NULL	gw70_molcellbiol_23_21_7648_s_228	14560010	(B) ChIp experiments documenting in vivo binding of Myc and Miz1 to DNA surrounding  the start site of transcription of the  P57KIP2and  P21CIP1 genes.	bind
8828	3	3727	6	11	NULL	NULL	NULL	Miz1	GP		bind					P57KIP2 gene	GP			DNA surrounding transcription start site	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7648_s_228	14560010	(B) ChIp experiments documenting in vivo binding of Myc and Miz1 to DNA surrounding  the start site of transcription of the  P57KIP2and  P21CIP1 genes.	bind
8829	4	3727	6	11	NULL	NULL	NULL	Miz1	GP		bind					p21Cip1	GP			DNA surrounding transcription start site	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7648_s_228	14560010	(B) ChIp experiments documenting in vivo binding of Myc and Miz1 to DNA surrounding  the start site of transcription of the  P57KIP2and  P21CIP1 genes.	bind
81426	1	3727	11	NULL	NULL	0	NULL	P57KIP2 gene	Gene		undergoes					transcription	MolecularProcess				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_21_7648_s_228	14560010	(B) ChIp experiments documenting in vivo binding of Myc and Miz1 to DNA surrounding  the start site of transcription of the  P57KIP2and  P21CIP1 genes.	bind
81427	2	3727	11	NULL	NULL	0	NULL	P21CIP1 gene	Gene		undergoes					transcription	MolecularProcess				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_21_7648_s_228	14560010	(B) ChIp experiments documenting in vivo binding of Myc and Miz1 to DNA surrounding  the start site of transcription of the  P57KIP2and  P21CIP1 genes.	bind
81428	3	3727	11	NULL	NULL	0	NULL	Myc	Protein		binds to 					P57KIP2 gene	Gene			transcription start site	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_21_7648_s_228	14560010	(B) ChIp experiments documenting in vivo binding of Myc and Miz1 to DNA surrounding  the start site of transcription of the  P57KIP2and  P21CIP1 genes.	bind
81429	4	3727	11	NULL	NULL	0	NULL	Myc	Protein		binds to 					P21CIP1 gene	Gene			transcription start site	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_21_7648_s_228	14560010	(B) ChIp experiments documenting in vivo binding of Myc and Miz1 to DNA surrounding  the start site of transcription of the  P57KIP2and  P21CIP1 genes.	bind
81430	5	3727	11	NULL	NULL	0	NULL	Miz1	Protein		binds to 					P57KIP2 gene	Gene			transcription start site	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_21_7648_s_228	14560010	(B) ChIp experiments documenting in vivo binding of Myc and Miz1 to DNA surrounding  the start site of transcription of the  P57KIP2and  P21CIP1 genes.	bind
81431	6	3727	11	NULL	NULL	0	NULL	Miz1	Gene		binds to 					P21CIP1 gene	Gene			transcription start site	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_21_7648_s_228	14560010	(B) ChIp experiments documenting in vivo binding of Myc and Miz1 to DNA surrounding  the start site of transcription of the  P57KIP2and  P21CIP1 genes.	bind
8647	1	3728	5	11	NULL	NULL	NULL	GATA-6	GP		bind									I-BRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6646_s_232	12944489	(B) ChIP of GATA-6 bound to I-BRE.	bind
8830	1	3728	6	11	NULL	NULL	NULL	GATA-6	GP		bind									I-BRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6646_s_232	12944489	(B) ChIP of GATA-6 bound to I-BRE.	bind
81432	1	3728	11	NULL	NULL	0	NULL	GATA-6	GeneOrProtein		binds to 					I-BRE	Gene				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_18_6646_s_232	12944489	(B) ChIP of GATA-6 bound to I-BRE.	bind
8648	1	3729	5	11	NULL	NULL	NULL	Smad1	GP		bind									BRE-1	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6646_s_161	12944489	(B) ChIP of Smad1 bound to BRE-1.	bind
8831	1	3729	6	11	NULL	NULL	NULL	Smad1	GP		bind									BRE-1	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6646_s_161	12944489	(B) ChIP of Smad1 bound to BRE-1.	bind
81433	1	3729	11	NULL	NULL	0	NULL	Smad1	GeneOrProtein		binds to 					BRE-1	Gene				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_18_6646_s_161	12944489	(B) ChIP of Smad1 bound to BRE-1.	bind
8649	1	3730	5	11	NULL	NULL	NULL	NF-Y	GP		bind					cyclin B2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_gene_312_0_225_s_254	12909359	(B) Chromatin immunoprecipitation (ChIP) assays showing binding of NF-Y to the  cyclin B2 promoter.	bind
8832	1	3730	6	11	NULL	NULL	NULL	NF-Y	GP		bind					cyclin B2 	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_gene_312_0_225_s_254	12909359	(B) Chromatin immunoprecipitation (ChIP) assays showing binding of NF-Y to the  cyclin B2 promoter.	bind
81434	1	3730	11	NULL	NULL	0	NULL	 NF-Y	GeneOrProtein		binds to 					cyclin B2	Gene			promoter	NULL		0	NULL	NULL	NULL	gw60_gene_312_0_225_s_254	12909359	(B) Chromatin immunoprecipitation (ChIP) assays showing binding of NF-Y to the  cyclin B2 promoter.	bind
8650	1	3731	5	11	NULL	NULL	NULL	Cks1	GP		bind					Skp2	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcell_7_3_639_s_181	11463388	(B) Cks1 binds Skp2 in vitro.	bind
8833	1	3731	6	11	NULL	NULL	NULL	Cks1	GP		bind					Skp2	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcell_7_3_639_s_181	11463388	(B) Cks1 binds Skp2 in vitro.	bind
81435	1	3731	11	NULL	NULL	0	NULL	Cks1	GeneOrProtein		binds to 					Skp2	GeneOrProtein				NULL	in vitro	0	NULL	NULL	NULL	gw60_molcell_7_3_639_s_181	11463388	(B) Cks1 binds Skp2 in vitro.	bind
8651	1	3733	5	11	NULL	NULL	NULL	EDA-A5	GP		bind					TROY receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_gene_371_1_42_s_111	16423472	(B) Co-immunoprecipitation analysis  for binding of EDA-A5  to TROY receptor.	bind
8834	1	3733	6	11	NULL	NULL	NULL	EDA-A5	GP		bind					TROY receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_gene_371_1_42_s_111	16423472	(B) Co-immunoprecipitation analysis  for binding of EDA-A5  to TROY receptor.	bind
81436	1	3733	11	NULL	NULL	0	NULL	EDA-A5	GeneOrProtein		binds to 					TROY receptor	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw70_gene_371_1_42_s_111	16423472	(B) Co-immunoprecipitation analysis  for binding of EDA-A5  to TROY receptor.	bind
8652	1	3734	5	11	NULL	NULL	NULL	CoA	GP		bind					CoaA protein	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_11_3410_s_125	12754240	(B) CoA binding of  CoaA protein mutants compared to that of wild-type CoaA.	bind
8653	2	3734	5	11	NULL	NULL	NULL	CoA	GP		bind					CoaA	GP	wild-type			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_11_3410_s_125	12754240	(B) CoA binding of  CoaA protein mutants compared to that of wild-type CoaA.	bind
8835	1	3734	6	11	NULL	NULL	NULL	CoA	GP		bind					CoaA protein	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_11_3410_s_125	12754240	(B) CoA binding of  CoaA protein mutants compared to that of wild-type CoaA.	bind
8989	2	3734	6	11	NULL	NULL	NULL	CoA	GP		bind					CoaA protein	GP	wild-type			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_11_3410_s_125	12754240	(B) CoA binding of  CoaA protein mutants compared to that of wild-type CoaA.	bind
8654	1	3736	5	11	NULL	NULL	NULL	Coatomer	GP		bind					Bet1p-GST	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_3_395_s_243	11970962	(B) Coatomer binds to Bet1p-GST via Glo3p.	bind
8655	2	3736	5	11	NULL	NULL	NULL	statement 1	Process		occurs via					Glo3p	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_3_395_s_243	11970962	(B) Coatomer binds to Bet1p-GST via Glo3p.	bind
9016	1	3736	6	11	NULL	NULL	NULL	Coatomer	GP		bind					Bet1p-GST	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_3_395_s_243	11970962	(B) Coatomer binds to Bet1p-GST via Glo3p.	bind
9017	2	3736	6	11	NULL	NULL	NULL	statement 1	Process		occurs via					Glo3p	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_3_395_s_243	11970962	(B) Coatomer binds to Bet1p-GST via Glo3p.	bind
81437	1	3736	11	NULL	NULL	0	NULL	Coatomer	Protein		binds to 					Bet1p-GST	Protein				NULL		0	NULL	NULL	NULL	gw60_cellbiol_157_3_395_s_243	11970962	(B) Coatomer binds to Bet1p-GST via Glo3p.	bind
81438	2	3736	11	NULL	NULL	0	NULL	Coatomer	Protein		binds to 					Glo3p	Protein				NULL		0	NULL	NULL	NULL	gw60_cellbiol_157_3_395_s_243	11970962	(B) Coatomer binds to Bet1p-GST via Glo3p.	bind
81439	3	3736	11	NULL	NULL	0	NULL	Glo3p	Protein		binds to 					Bet1p-GST	Protein				NULL		0	NULL	NULL	NULL	gw60_cellbiol_157_3_395_s_243	11970962	(B) Coatomer binds to Bet1p-GST via Glo3p.	bind
8656	2	3737	5	11	NULL	NULL	NULL	K2-3f	GP		bind			scFv		statement 1	Cell				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1638_3_257_s_277	12878327	(B) Cocaine  inhibition of scFv K2-3f binding to the hDAT expressed on the surface of a transfected  neuroblastoma N1E-115 cell line.	bind
8657	3	3737	5	11	NULL	NULL	NULL	Cocaine	Chemical		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1638_3_257_s_277	12878327	(B) Cocaine  inhibition of scFv K2-3f binding to the hDAT expressed on the surface of a transfected  neuroblastoma N1E-115 cell line.	bind
10029	1	3737	5	11	NULL	NULL	NULL	hDAT	GP		expressed					on surface of neuroblastoma N1E-115 cells	Cell	transfected			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1638_3_257_s_277	12878327	(B) Cocaine  inhibition of scFv K2-3f binding to the hDAT expressed on the surface of a transfected  neuroblastoma N1E-115 cell line.	bind
9018	1	3737	6	11	NULL	NULL	NULL	 K2-3f	GP		bind			scFv		hDAT	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1638_3_257_s_277	12878327	(B) Cocaine  inhibition of scFv K2-3f binding to the hDAT expressed on the surface of a transfected  neuroblastoma N1E-115 cell line.	bind
9019	2	3737	6	11	NULL	NULL	NULL	hDAT	GP		expressed on 					neuroblastoma N1E-115 cell line	Cell	surface of transfected			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1638_3_257_s_277	12878327	(B) Cocaine  inhibition of scFv K2-3f binding to the hDAT expressed on the surface of a transfected  neuroblastoma N1E-115 cell line.	bind
53475	3	3737	6	11	NULL	NULL	NULL	Cocaine	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1638_3_257_s_277	12878327	(B) Cocaine  inhibition of scFv K2-3f binding to the hDAT expressed on the surface of a transfected  neuroblastoma N1E-115 cell line.	bind
81440	1	3737	11	NULL	NULL	0	NULL	scFv K2-3f	GeneOrProtein		binds to 					hDAT	GeneOrProtein	 neuroblastoma;;N1E-115 cell line			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1638_3_257_s_277	12878327	(B) Cocaine  inhibition of scFv K2-3f binding to the hDAT expressed on the surface of a transfected  neuroblastoma N1E-115 cell line.	bind
81441	2	3737	11	NULL	NULL	0	NULL	Cocaine	NonProteinOrNucleicAcidChemical		inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1638_3_257_s_277	12878327	(B) Cocaine  inhibition of scFv K2-3f binding to the hDAT expressed on the surface of a transfected  neuroblastoma N1E-115 cell line.	bind
8658	1	3740	5	11	NULL	NULL	NULL	Cdc50p-GFP	GP		colocalize with					myc-Vps21p	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_2_730_s_248	12589066	(B) Colocalization of Cdc50p-GFP with myc-Vps21p.	bind
9020	1	3740	6	11	NULL	NULL	NULL	Cdc50p-GFP	GP		colocalizes with					myc-Vps21p	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_2_730_s_248	12589066	(B) Colocalization of Cdc50p-GFP with myc-Vps21p.	bind
81442	1	3740	11	NULL	NULL	0	NULL	Cdc50p-GFP	GeneOrProtein		colocalizes with					myc-Vps21p	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_2_730_s_248	12589066	(B) Colocalization of Cdc50p-GFP with myc-Vps21p.	bind
81443	1	3743	11	NULL	NULL	0	NULL	 leucine	AminoAcid		binds to 					BacA	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_9_4509_s_111	12200307	(B) Comparison of one of the three leucine-specific consensus sequences found in the leucine binding domains of BacA, LicA, LchAA, LicB, LchAB, SrfAA, and SrfAB ( 52) with the corresponding residues in the sequenced part of amphisin synthetase.	bind
81444	2	3743	11	NULL	NULL	0	NULL	 leucine	AminoAcid		binds to 					LicA	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_9_4509_s_111	12200307	(B) Comparison of one of the three leucine-specific consensus sequences found in the leucine binding domains of BacA, LicA, LchAA, LicB, LchAB, SrfAA, and SrfAB ( 52) with the corresponding residues in the sequenced part of amphisin synthetase.	bind
81445	3	3743	11	NULL	NULL	0	NULL	leucine	AminoAcid		binds to 					LchAA	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_9_4509_s_111	12200307	(B) Comparison of one of the three leucine-specific consensus sequences found in the leucine binding domains of BacA, LicA, LchAA, LicB, LchAB, SrfAA, and SrfAB ( 52) with the corresponding residues in the sequenced part of amphisin synthetase.	bind
81446	4	3743	11	NULL	NULL	0	NULL	leucine	AminoAcid		binds to 					LicB	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_9_4509_s_111	12200307	(B) Comparison of one of the three leucine-specific consensus sequences found in the leucine binding domains of BacA, LicA, LchAA, LicB, LchAB, SrfAA, and SrfAB ( 52) with the corresponding residues in the sequenced part of amphisin synthetase.	bind
81447	5	3743	11	NULL	NULL	0	NULL	leucine	AminoAcid		binds to 					LchAB	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_9_4509_s_111	12200307	(B) Comparison of one of the three leucine-specific consensus sequences found in the leucine binding domains of BacA, LicA, LchAA, LicB, LchAB, SrfAA, and SrfAB ( 52) with the corresponding residues in the sequenced part of amphisin synthetase.	bind
81448	6	3743	11	NULL	NULL	0	NULL	leucine	AminoAcid		binds to 					SrfAA	Gene				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_9_4509_s_111	12200307	(B) Comparison of one of the three leucine-specific consensus sequences found in the leucine binding domains of BacA, LicA, LchAA, LicB, LchAB, SrfAA, and SrfAB ( 52) with the corresponding residues in the sequenced part of amphisin synthetase.	bind
81449	7	3743	11	NULL	NULL	0	NULL	leucine	AminoAcid		binds to 					SrfAB	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_9_4509_s_111	12200307	(B) Comparison of one of the three leucine-specific consensus sequences found in the leucine binding domains of BacA, LicA, LchAA, LicB, LchAB, SrfAA, and SrfAB ( 52) with the corresponding residues in the sequenced part of amphisin synthetase.	bind
8659	2	3744	5	11	NULL	NULL	NULL	PCAF	GP		bind			bromodomain		statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_9_3_575_s_37	11931765	(B) Comparison of PCAF bromodomain binding to lysine-acetylated peptide derived from HIV-1 Tat at K50 (SYGR-AcK-KRRQR) (left) versus one derived from histone H4 at K16 (SGRGKGGKGLGKGGA-AcK-RHRK) (right).	bind
8660	4	3744	5	11	NULL	NULL	NULL	PCAF	GP		bind			bromodomain		statement 3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_9_3_575_s_37	11931765	(B) Comparison of PCAF bromodomain binding to lysine-acetylated peptide derived from HIV-1 Tat at K50 (SYGR-AcK-KRRQR) (left) versus one derived from histone H4 at K16 (SGRGKGGKGLGKGGA-AcK-RHRK) (right).	bind
10024	1	3744	5	11	NULL	NULL	NULL	peptide	GP	acetylated	derived from			lysine		HIV-1 Tat	GP		k50(SYGR-AcK-KRRQR)		NULL		NULL	NULL	NULL	NULL	gw60_molcell_9_3_575_s_37	11931765	(B) Comparison of PCAF bromodomain binding to lysine-acetylated peptide derived from HIV-1 Tat at K50 (SYGR-AcK-KRRQR) (left) versus one derived from histone H4 at K16 (SGRGKGGKGLGKGGA-AcK-RHRK) (right).	bind
10025	3	3744	5	11	NULL	NULL	NULL	peptide	GP	acetylated	derived from			lysine		histone H4	GP		K16 (SGRGKGGKGLGKGGA-AcK-RHRK)		NULL		NULL	NULL	NULL	NULL	gw60_molcell_9_3_575_s_37	11931765	(B) Comparison of PCAF bromodomain binding to lysine-acetylated peptide derived from HIV-1 Tat at K50 (SYGR-AcK-KRRQR) (left) versus one derived from histone H4 at K16 (SGRGKGGKGLGKGGA-AcK-RHRK) (right).	bind
9021	1	3744	6	11	NULL	NULL	NULL	 peptide	GP	acetylated	derived from			lysine		HIV-1-Tat	GP		K50 (SYGR-AcK-KRRQR)		NULL		NULL	NULL	NULL	NULL	gw60_molcell_9_3_575_s_37	11931765	(B) Comparison of PCAF bromodomain binding to lysine-acetylated peptide derived from HIV-1 Tat at K50 (SYGR-AcK-KRRQR) (left) versus one derived from histone H4 at K16 (SGRGKGGKGLGKGGA-AcK-RHRK) (right).	bind
9022	2	3744	6	11	NULL	NULL	NULL	peptide	GP	acetylated 	derived from			lysine		histone H4	GP		K16 (SGRGKGGKGLGKGGA-AcK-RHRK)		NULL		NULL	NULL	NULL	NULL	gw60_molcell_9_3_575_s_37	11931765	(B) Comparison of PCAF bromodomain binding to lysine-acetylated peptide derived from HIV-1 Tat at K50 (SYGR-AcK-KRRQR) (left) versus one derived from histone H4 at K16 (SGRGKGGKGLGKGGA-AcK-RHRK) (right).	bind
9023	3	3744	6	11	NULL	NULL	NULL	PCAF	GP		bind			bromodomain		statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_9_3_575_s_37	11931765	(B) Comparison of PCAF bromodomain binding to lysine-acetylated peptide derived from HIV-1 Tat at K50 (SYGR-AcK-KRRQR) (left) versus one derived from histone H4 at K16 (SGRGKGGKGLGKGGA-AcK-RHRK) (right).	bind
9024	4	3744	6	11	NULL	NULL	NULL	PCAF	GP		bind			bromodomain		statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_9_3_575_s_37	11931765	(B) Comparison of PCAF bromodomain binding to lysine-acetylated peptide derived from HIV-1 Tat at K50 (SYGR-AcK-KRRQR) (left) versus one derived from histone H4 at K16 (SGRGKGGKGLGKGGA-AcK-RHRK) (right).	bind
81450	1	3744	11	NULL	NULL	0	NULL	PCAF 	Protein		binds to 			bromodomain		lysine-acetylated peptide	PartOfProtein	HIV-1 Tat			NULL		0	NULL	NULL	NULL	gw60_molcell_9_3_575_s_37	11931765	(B) Comparison of PCAF bromodomain binding to lysine-acetylated peptide derived from HIV-1 Tat at K50 (SYGR-AcK-KRRQR) (left) versus one derived from histone H4 at K16 (SGRGKGGKGLGKGGA-AcK-RHRK) (right).	bind
8661	1	3745	5	11	NULL	NULL	NULL	H-NS	GP		bind					PCR fragments	NucleicAcid	representing -310 fusion			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_22_6497_s_197	14594821	(B) Comparison of the binding of H-NS to PCR fragments representing the  -310 and -310d4 fusions.	bind
8662	2	3745	5	11	NULL	NULL	NULL	H-NS	GP		bind					PCR fragments	NucleicAcid	representing -310d4 fusion			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_22_6497_s_197	14594821	(B) Comparison of the binding of H-NS to PCR fragments representing the  -310 and -310d4 fusions.	bind
9025	1	3745	6	11	NULL	NULL	NULL	H-NS	GP		bind					PCR fragments	NucleicAcid	-310 fusions			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_22_6497_s_197	14594821	(B) Comparison of the binding of H-NS to PCR fragments representing the  -310 and -310d4 fusions.	bind
9699	2	3745	6	11	NULL	NULL	NULL	H-NS	GP		bind					PCR fragments	NucleicAcid	-310d4 fusions			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_22_6497_s_197	14594821	(B) Comparison of the binding of H-NS to PCR fragments representing the  -310 and -310d4 fusions.	bind
81451	1	3745	11	NULL	NULL	0	NULL	 H-NS	GeneOrProtein		binds to 					PCR fragment	PartOfProtein				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_22_6497_s_197	14594821	(B) Comparison of the binding of H-NS to PCR fragments representing the  -310 and -310d4 fusions.	bind
8663	1	3747	5	11	NULL	NULL	NULL	L1 lipid	Chemical		bind		tightly			sIgA	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1735_3_153_s_213	16039903	(B) Comparison of the incorporation of 32P label into L1 and L2 lipids tightly bound to sIgA by TLC on a Kieselgel plates using  chloroform-methanol-7 M NH4OH (60:35:5).	bind
8664	2	3747	5	11	NULL	NULL	NULL	L2 lipid	Chemical		bind		tightly			sIgA	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1735_3_153_s_213	16039903	(B) Comparison of the incorporation of 32P label into L1 and L2 lipids tightly bound to sIgA by TLC on a Kieselgel plates using  chloroform-methanol-7 M NH4OH (60:35:5).	bind
9026	1	3747	6	11	NULL	NULL	NULL	L1 lipid	Chemical		bind		tightly			sIgA	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1735_3_153_s_213	16039903	(B) Comparison of the incorporation of 32P label into L1 and L2 lipids tightly bound to sIgA by TLC on a Kieselgel plates using  chloroform-methanol-7 M NH4OH (60:35:5).	bind
9027	2	3747	6	11	NULL	NULL	NULL	L2 lipid	Chemical		bind		tightly			sIgA	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1735_3_153_s_213	16039903	(B) Comparison of the incorporation of 32P label into L1 and L2 lipids tightly bound to sIgA by TLC on a Kieselgel plates using  chloroform-methanol-7 M NH4OH (60:35:5).	bind
81452	1	3747	11	NULL	NULL	0	NULL	L1 lipid	NonProteinOrNucleicAcidChemical		binds to 		tightly			sIgA	Protein				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1735_3_153_s_213	16039903	(B) Comparison of the incorporation of 32P label into L1 and L2 lipids tightly bound to sIgA by TLC on a Kieselgel plates using  chloroform-methanol-7 M NH4OH (60:35:5).	bind
81453	2	3747	11	NULL	NULL	NULL	NULL	L2 lipid	NonProteinOrNucleicAcidChemical		binds to 		tightly			sIgA	Protein				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1735_3_153_s_213	16039903	(B) Comparison of the incorporation of 32P label into L1 and L2 lipids tightly bound to sIgA by TLC on a Kieselgel plates using  chloroform-methanol-7 M NH4OH (60:35:5).	bind
8665	1	3750	5	11	NULL	NULL	NULL	Mcm1	GP		bind					ARS120	NucleicAcid		fragment I		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_14_6514_s_215	15226450	(B) Competition  for binding of Mcm1 by fragment I of ARS120 and ARS131a.	bind
8666	2	3750	5	11	NULL	NULL	NULL	Mcm1	GP		bind					ARS131a	NucleicAcid		fragment I		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_14_6514_s_215	15226450	(B) Competition  for binding of Mcm1 by fragment I of ARS120 and ARS131a.	bind
8667	3	3750	5	11	NULL	NULL	NULL	statement 1	Process		compete with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_14_6514_s_215	15226450	(B) Competition  for binding of Mcm1 by fragment I of ARS120 and ARS131a.	bind
9414	1	3750	6	11	NULL	NULL	NULL	Mcm1	GP		bind					ARS120	NucleicAcid		fragment 1 		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_14_6514_s_215	15226450	(B) Competition  for binding of Mcm1 by fragment I of ARS120 and ARS131a.	bind
9415	2	3750	6	11	NULL	NULL	NULL	Mcm1	GP		bind					ARS131a	NucleicAcid		fragment 1 		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_14_6514_s_215	15226450	(B) Competition  for binding of Mcm1 by fragment I of ARS120 and ARS131a.	bind
9416	3	3750	6	11	NULL	NULL	NULL	statement 1	Process		competes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_14_6514_s_215	15226450	(B) Competition  for binding of Mcm1 by fragment I of ARS120 and ARS131a.	bind
81454	1	3750	11	NULL	NULL	0	NULL	 Mcm1	GeneOrProtein		binds to 					fragment I	NucleicAcidSubstance	ARS120			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_14_6514_s_215	15226450	(B) Competition  for binding of Mcm1 by fragment I of ARS120 and ARS131a.	bind
81455	2	3750	11	NULL	NULL	0	NULL	Mcm1	GeneOrProtein		binds to 					fragment I	NucleicAcidSubstance	ARS131a			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_14_6514_s_215	15226450	(B) Competition  for binding of Mcm1 by fragment I of ARS120 and ARS131a.	bind
8668	1	3751	5	11	NULL	NULL	NULL	gp120	GP	biotinylated;; HIV-1	bind					DC-SIGN	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_5_653_s_181	12433371	(B) Competition assay of biotinylated HIV-1 gp120 binding to DC-SIGN.	bind
9028	1	3751	6	11	NULL	NULL	NULL	gp120	GP	biotinylated;; HIV-1	bind					DC-SIGN	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_5_653_s_181	12433371	(B) Competition assay of biotinylated HIV-1 gp120 binding to DC-SIGN.	bind
81456	1	3751	11	NULL	NULL	0	NULL	gp120	GeneOrProtein	HIV-1;;biotinylated	binds to 					DC-SIGN	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_immunity_17_5_653_s_181	12433371	(B) Competition assay of biotinylated HIV-1 gp120 binding to DC-SIGN.	bind
8669	1	3753	5	11	NULL	NULL	NULL	C/EBPdelta	GP		bind				APRE	Stat3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2108_s_244	9528783	(B) Competition for Stat3 binding by the C/EBPdelta APRE.	bind
9029	1	3753	6	11	NULL	NULL	NULL	Stat3	GP		bind					C/EBPdelta	GP			APRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2108_s_244	9528783	(B) Competition for Stat3 binding by the C/EBPdelta APRE.	bind
81457	1	3753	11	NULL	NULL	0	NULL	C/EBPdelta	Gene		binds to 				APRE	Stat3	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_4_2108_s_244	9528783	(B) Competition for Stat3 binding by the C/EBPdelta APRE.	bind
8879	1	3754	5	11	NULL	NULL	NULL	p53	GP		bind					PUMA	GP			 binding site 2	NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_683_s_94	11463392	(B) Competitive inhibition of p53 binding to the PUMA binding site 2 with the wild-type PUMA BS2 but not the mutant PUMA BS2 oligonucleotide	bind
8881	2	3754	5	11	NULL	NULL	NULL	p53	GP		bind					PUMA	GP	wild-type		BS2	NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_683_s_94	11463392	(B) Competitive inhibition of p53 binding to the PUMA binding site 2 with the wild-type PUMA BS2 but not the mutant PUMA BS2 oligonucleotide	bind
8882	3	3754	5	11	NULL	NULL	NULL	statement 2	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_683_s_94	11463392	(B) Competitive inhibition of p53 binding to the PUMA binding site 2 with the wild-type PUMA BS2 but not the mutant PUMA BS2 oligonucleotide	bind
8883	4	3754	5	11	NULL	NULL	NULL	p53	GP		does not bind					PUMA	GP	mutant		BS2 oligonucleotide	NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_683_s_94	11463392	(B) Competitive inhibition of p53 binding to the PUMA binding site 2 with the wild-type PUMA BS2 but not the mutant PUMA BS2 oligonucleotide	bind
8884	5	3754	5	11	NULL	NULL	NULL	statement 4	Process		does not compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_683_s_94	11463392	(B) Competitive inhibition of p53 binding to the PUMA binding site 2 with the wild-type PUMA BS2 but not the mutant PUMA BS2 oligonucleotide	bind
9030	1	3754	6	11	NULL	NULL	NULL	p53	GP		bind					PUMA	GP			binding site 2	NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_683_s_94	11463392	(B) Competitive inhibition of p53 binding to the PUMA binding site 2 with the wild-type PUMA BS2 but not the mutant PUMA BS2 oligonucleotide	bind
9031	2	3754	6	11	NULL	NULL	NULL	p53	GP		bind					PUMA	GP	wild-type		BS2	NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_683_s_94	11463392	(B) Competitive inhibition of p53 binding to the PUMA binding site 2 with the wild-type PUMA BS2 but not the mutant PUMA BS2 oligonucleotide	bind
9032	3	3754	6	11	NULL	NULL	NULL	statement 1	Process		competes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_683_s_94	11463392	(B) Competitive inhibition of p53 binding to the PUMA binding site 2 with the wild-type PUMA BS2 but not the mutant PUMA BS2 oligonucleotide	bind
9033	4	3754	6	11	NULL	NULL	NULL	p53	GP		does not bind					PUMA 	GP	mutant		BS2  oligonucletide	NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_683_s_94	11463392	(B) Competitive inhibition of p53 binding to the PUMA binding site 2 with the wild-type PUMA BS2 but not the mutant PUMA BS2 oligonucleotide	bind
53476	5	3754	6	11	NULL	NULL	NULL	statement 4	Process		does not compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_683_s_94	11463392	(B) Competitive inhibition of p53 binding to the PUMA binding site 2 with the wild-type PUMA BS2 but not the mutant PUMA BS2 oligonucleotide	bind
81458	1	3754	11	NULL	NULL	NULL	NULL	 p53	GeneOrProtein		binds to 					PUMA	GeneOrProtein				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_683_s_94	11463392	(B) Competitive inhibition of p53 binding to the PUMA binding site 2 with the wild-type PUMA BS2 but not the mutant PUMA BS2 oligonucleotide	bind
81459	2	3754	11	NULL	NULL	NULL	NULL	PUMA BS2	GeneOrProtein	wild-type	Competitively inhibit					PUMA	GeneOrProtein	binding site 2			NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_683_s_94	11463392	(B) Competitive inhibition of p53 binding to the PUMA binding site 2 with the wild-type PUMA BS2 but not the mutant PUMA BS2 oligonucleotide	bind
81460	3	3754	11	NULL	NULL	0	NULL	PUMA BS2	NucleicAcidSubstance	mutant	Competitively inhibit					PUMA	GeneOrProtein	binding site 2			NULL		0	NULL	NULL	NULL	gw60_molcell_7_3_683_s_94	11463392	(B) Competitive inhibition of p53 binding to the PUMA binding site 2 with the wild-type PUMA BS2 but not the mutant PUMA BS2 oligonucleotide	bind
8670	1	3755	5	11	NULL	NULL	NULL	Complexin	GP		bind					ternary SNARE complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_283_s_158	16267273	(B) Complexin binding to the ternary SNARE complex.	bind
9034	1	3755	6	11	NULL	NULL	NULL	Complexin	GP		bind					ternary SNARE complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_283_s_158	16267273	(B) Complexin binding to the ternary SNARE complex.	bind
81461	1	3755	11	NULL	NULL	0	NULL	Complexin	GeneOrProtein		binds to 					SNARE	Protein	ternary complex			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_1_283_s_158	16267273	(B) Complexin binding to the ternary SNARE complex.	bind
8671	1	3756	5	11	NULL	NULL	NULL	KorB (pSB24.2)	GP		bind					pIJ101 kilB	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_13_3780_s_110	12813071	(B) Concentration-dependent characteristics of KorB (pSB24.2) binding  to the pIJ101  kilB promoter.	bind
8672	2	3756	5	11	NULL	NULL	NULL	statement 1	Process		is dependent on					concentration	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_13_3780_s_110	12813071	(B) Concentration-dependent characteristics of KorB (pSB24.2) binding  to the pIJ101  kilB promoter.	bind
9035	1	3756	6	11	NULL	NULL	NULL	KorB (pSB24.2)	GP		bind					pIJ101 kilB	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_13_3780_s_110	12813071	(B) Concentration-dependent characteristics of KorB (pSB24.2) binding  to the pIJ101  kilB promoter.	bind
53477	2	3756	6	11	NULL	NULL	NULL	statement 1	Process		depends on					Concentration	QuantityOrMeasure				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_13_3780_s_110	12813071	(B) Concentration-dependent characteristics of KorB (pSB24.2) binding  to the pIJ101  kilB promoter.	bind
81462	1	3756	11	NULL	NULL	0	NULL	KorB	GeneOrProtein		binds to 					pIJ101 kilB	Gene			promoter	NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_13_3780_s_110	12813071	(B) Concentration-dependent characteristics of KorB (pSB24.2) binding  to the pIJ101  kilB promoter.	bind
8673	1	3758	5	11	NULL	NULL	NULL	GTP S	NucleicAcid		bind					MBP-T43NTR-Gi	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_493_2_101_s_104	11287004	(B) Concentration-response curves for NT-induced [35]GTP S binding to MBP-T43NTR-Gi (squares) or MBP-T43NTR-Gi/q (triangles).	bind
8674	2	3758	5	11	NULL	NULL	NULL	NT	GP		induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_493_2_101_s_104	11287004	(B) Concentration-response curves for NT-induced [35]GTP S binding to MBP-T43NTR-Gi (squares) or MBP-T43NTR-Gi/q (triangles).	bind
8675	3	3758	5	11	NULL	NULL	NULL	GTP S	NucleicAcid		bind					MBP-T43NTR-Gi/q	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_493_2_101_s_104	11287004	(B) Concentration-response curves for NT-induced [35]GTP S binding to MBP-T43NTR-Gi (squares) or MBP-T43NTR-Gi/q (triangles).	bind
8676	4	3758	5	11	NULL	NULL	NULL	NT	GP		induce					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_493_2_101_s_104	11287004	(B) Concentration-response curves for NT-induced [35]GTP S binding to MBP-T43NTR-Gi (squares) or MBP-T43NTR-Gi/q (triangles).	bind
53478	5	3758	5	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_493_2_101_s_104	11287004	(B) Concentration-response curves for NT-induced [35]GTP S binding to MBP-T43NTR-Gi (squares) or MBP-T43NTR-Gi/q (triangles).	bind
9036	1	3758	6	11	NULL	NULL	NULL	GTP S	NucleicAcid		bind					MBP-T43NTR-Gi	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_493_2_101_s_104	11287004	(B) Concentration-response curves for NT-induced [35]GTP S binding to MBP-T43NTR-Gi (squares) or MBP-T43NTR-Gi/q (triangles).	bind
9037	2	3758	6	11	NULL	NULL	NULL	GTP S	NucleicAcid		bind					MBP-T43NTR-Gi/q	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_493_2_101_s_104	11287004	(B) Concentration-response curves for NT-induced [35]GTP S binding to MBP-T43NTR-Gi (squares) or MBP-T43NTR-Gi/q (triangles).	bind
9038	3	3758	6	11	NULL	NULL	NULL	NT	GP		induces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_493_2_101_s_104	11287004	(B) Concentration-response curves for NT-induced [35]GTP S binding to MBP-T43NTR-Gi (squares) or MBP-T43NTR-Gi/q (triangles).	bind
9039	4	3758	6	11	NULL	NULL	NULL	NT	GP		induces					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_493_2_101_s_104	11287004	(B) Concentration-response curves for NT-induced [35]GTP S binding to MBP-T43NTR-Gi (squares) or MBP-T43NTR-Gi/q (triangles).	bind
9040	5	3758	6	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_493_2_101_s_104	11287004	(B) Concentration-response curves for NT-induced [35]GTP S binding to MBP-T43NTR-Gi (squares) or MBP-T43NTR-Gi/q (triangles).	bind
81463	1	3758	11	NULL	NULL	0	NULL	GTP	NonProteinOrNucleicAcidChemical		binds to 					MBP-T43NTR-Gi	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_febslett_493_2_101_s_104	11287004	(B) Concentration-response curves for NT-induced [35]GTP S binding to MBP-T43NTR-Gi (squares) or MBP-T43NTR-Gi/q (triangles).	bind
81464	2	3758	11	NULL	NULL	0	NULL	GTP	Chemical		binds to 					MBP-T43NTR-Gi/q	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_febslett_493_2_101_s_104	11287004	(B) Concentration-response curves for NT-induced [35]GTP S binding to MBP-T43NTR-Gi (squares) or MBP-T43NTR-Gi/q (triangles).	bind
81465	3	3758	11	NULL	NULL	0	NULL	NT	PartOfProtein		induces					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_493_2_101_s_104	11287004	(B) Concentration-response curves for NT-induced [35]GTP S binding to MBP-T43NTR-Gi (squares) or MBP-T43NTR-Gi/q (triangles).	bind
81466	4	3758	11	NULL	NULL	0	NULL	NT	PartOfProtein		induces					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_493_2_101_s_104	11287004	(B) Concentration-response curves for NT-induced [35]GTP S binding to MBP-T43NTR-Gi (squares) or MBP-T43NTR-Gi/q (triangles).	bind
8677	1	3762	5	11	NULL	NULL	NULL	IRF-3	GP		bind					IFNA1	GP			VRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_16_5721_s_400	12138184	(B) Cooperation between IRF-3 and IRF-5 binding to IFNA1 VRE enhances IRF-5-induced IFNA1 expression.	bind
8678	2	3762	5	11	NULL	NULL	NULL	IRF-5	GP		bind					IFNA1	GP			VRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_16_5721_s_400	12138184	(B) Cooperation between IRF-3 and IRF-5 binding to IFNA1 VRE enhances IRF-5-induced IFNA1 expression.	bind
8679	3	3762	5	11	NULL	NULL	NULL	statement 1	Process		occurs in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_16_5721_s_400	12138184	(B) Cooperation between IRF-3 and IRF-5 binding to IFNA1 VRE enhances IRF-5-induced IFNA1 expression.	bind
8680	4	3762	5	11	NULL	NULL	NULL	IRF-5	GP		induce					IFNA1	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_16_5721_s_400	12138184	(B) Cooperation between IRF-3 and IRF-5 binding to IFNA1 VRE enhances IRF-5-induced IFNA1 expression.	bind
8681	5	3762	5	11	NULL	NULL	NULL	statement 3	Process		enhances					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_16_5721_s_400	12138184	(B) Cooperation between IRF-3 and IRF-5 binding to IFNA1 VRE enhances IRF-5-induced IFNA1 expression.	bind
9041	1	3762	6	11	NULL	NULL	NULL	IRF-3	GP		bind					IFNA1	GP			VRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_16_5721_s_400	12138184	(B) Cooperation between IRF-3 and IRF-5 binding to IFNA1 VRE enhances IRF-5-induced IFNA1 expression.	bind
9042	2	3762	6	11	NULL	NULL	NULL	IRF-5	GP		bind					IFNA1	GP			VRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_16_5721_s_400	12138184	(B) Cooperation between IRF-3 and IRF-5 binding to IFNA1 VRE enhances IRF-5-induced IFNA1 expression.	bind
9043	3	3762	6	11	NULL	NULL	NULL	statement 1	Process		occurs in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_16_5721_s_400	12138184	(B) Cooperation between IRF-3 and IRF-5 binding to IFNA1 VRE enhances IRF-5-induced IFNA1 expression.	bind
9044	4	3762	6	11	NULL	NULL	NULL	IRF-5	GP		induces					IFNA1	GP	expression of 			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_16_5721_s_400	12138184	(B) Cooperation between IRF-3 and IRF-5 binding to IFNA1 VRE enhances IRF-5-induced IFNA1 expression.	bind
9045	5	3762	6	11	NULL	NULL	NULL	statement 3	Process		enhances					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_16_5721_s_400	12138184	(B) Cooperation between IRF-3 and IRF-5 binding to IFNA1 VRE enhances IRF-5-induced IFNA1 expression.	bind
81467	1	3762	11	NULL	NULL	0	NULL	 IRF-3 	GeneOrProtein		binds to 					IFNA1	Gene			VRE	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_16_5721_s_400	12138184	(B) Cooperation between IRF-3 and IRF-5 binding to IFNA1 VRE enhances IRF-5-induced IFNA1 expression.	bind
81468	2	3762	11	NULL	NULL	0	NULL	IRF-5 	GeneOrProtein		binds to 					IFNA1	Gene			VRE	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_16_5721_s_400	12138184	(B) Cooperation between IRF-3 and IRF-5 binding to IFNA1 VRE enhances IRF-5-induced IFNA1 expression.	bind
81469	3	3762	11	NULL	NULL	0	NULL	IRF-3	GeneOrProtein		Cooperate with					IRF-5	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_16_5721_s_400	12138184	(B) Cooperation between IRF-3 and IRF-5 binding to IFNA1 VRE enhances IRF-5-induced IFNA1 expression.	bind
81470	4	3762	11	NULL	NULL	0	NULL	IRF-5	GeneOrProtein		induces					IFNA1	Gene	expression			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_16_5721_s_400	12138184	(B) Cooperation between IRF-3 and IRF-5 binding to IFNA1 VRE enhances IRF-5-induced IFNA1 expression.	bind
81471	5	3762	11	NULL	NULL	0	NULL	statement 1	Process		enhances					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_16_5721_s_400	12138184	(B) Cooperation between IRF-3 and IRF-5 binding to IFNA1 VRE enhances IRF-5-induced IFNA1 expression.	bind
81472	6	3762	11	NULL	NULL	0	NULL	statement 2	Process		enhances					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_16_5721_s_400	12138184	(B) Cooperation between IRF-3 and IRF-5 binding to IFNA1 VRE enhances IRF-5-induced IFNA1 expression.	bind
8682	1	3764	5	11	NULL	NULL	NULL	SF-1	GP	COS1-overexpressed	bind					PE1 probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_9_3492_s_146	15831456	(B) COS1-overexpressed SF-1 and  LRH-1 binding to the PE1, PE2, and DR0 probes in the absence or presence of antibodies.	bind
8683	2	3764	5	11	NULL	NULL	NULL	LRH-1	GP	COS1-overexpressed	bind					PE1 probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_9_3492_s_146	15831456	(B) COS1-overexpressed SF-1 and  LRH-1 binding to the PE1, PE2, and DR0 probes in the absence or presence of antibodies.	bind
8684	3	3764	5	11	NULL	NULL	NULL	SF-1	GP	COS1-overexpressed	bind					PE2 probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_9_3492_s_146	15831456	(B) COS1-overexpressed SF-1 and  LRH-1 binding to the PE1, PE2, and DR0 probes in the absence or presence of antibodies.	bind
8685	4	3764	5	11	NULL	NULL	NULL	LRH-1	GP	COS1-overexpressed	bind					PE2 probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_9_3492_s_146	15831456	(B) COS1-overexpressed SF-1 and  LRH-1 binding to the PE1, PE2, and DR0 probes in the absence or presence of antibodies.	bind
8686	5	3764	5	11	NULL	NULL	NULL	SF-1	GP	COS1-overexpressed	bind					DRO probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_9_3492_s_146	15831456	(B) COS1-overexpressed SF-1 and  LRH-1 binding to the PE1, PE2, and DR0 probes in the absence or presence of antibodies.	bind
8687	6	3764	5	11	NULL	NULL	NULL	LRH-1	GP	COS1-overexpressed	bind					DRO probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_9_3492_s_146	15831456	(B) COS1-overexpressed SF-1 and  LRH-1 binding to the PE1, PE2, and DR0 probes in the absence or presence of antibodies.	bind
9046	1	3764	6	11	NULL	NULL	NULL	SF-1	GP	COS-1 overexpressed	bind					PE1 probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_9_3492_s_146	15831456	(B) COS1-overexpressed SF-1 and  LRH-1 binding to the PE1, PE2, and DR0 probes in the absence or presence of antibodies.	bind
9048	2	3764	6	11	NULL	NULL	NULL	SF-1	GP	COS-1 overexpressed	bind					PE2 probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_9_3492_s_146	15831456	(B) COS1-overexpressed SF-1 and  LRH-1 binding to the PE1, PE2, and DR0 probes in the absence or presence of antibodies.	bind
9049	3	3764	6	11	NULL	NULL	NULL	SF-1	GP	COS-1 overexpressed	bind					DR0 probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_9_3492_s_146	15831456	(B) COS1-overexpressed SF-1 and  LRH-1 binding to the PE1, PE2, and DR0 probes in the absence or presence of antibodies.	bind
9050	4	3764	6	11	NULL	NULL	NULL	LRH-1	GP	COS-1 overexpressed	bind					PE1 probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_9_3492_s_146	15831456	(B) COS1-overexpressed SF-1 and  LRH-1 binding to the PE1, PE2, and DR0 probes in the absence or presence of antibodies.	bind
9051	5	3764	6	11	NULL	NULL	NULL	LRH-1	GP	COS-1 overexpressed	bind					PE2 probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_9_3492_s_146	15831456	(B) COS1-overexpressed SF-1 and  LRH-1 binding to the PE1, PE2, and DR0 probes in the absence or presence of antibodies.	bind
9052	6	3764	6	11	NULL	NULL	NULL	LRH-1	GP	COS-1 overexpressed	bind					DR0 probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_9_3492_s_146	15831456	(B) COS1-overexpressed SF-1 and  LRH-1 binding to the PE1, PE2, and DR0 probes in the absence or presence of antibodies.	bind
81473	1	3764	11	NULL	NULL	NULL	NULL	SF-1	GeneOrProtein	COS1-overexpressed	binds to 					PE1 probe	NucleicAcidSubstance				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_9_3492_s_146	15831456	(B) COS1-overexpressed SF-1 and  LRH-1 binding to the PE1, PE2, and DR0 probes in the absence or presence of antibodies.	bind
81474	2	3764	11	NULL	NULL	NULL	NULL	 LRH-1	GeneOrProtein	COS1-overexpressed	binds to 					PE1 probe	NucleicAcidSubstance				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_9_3492_s_146	15831456	(B) COS1-overexpressed SF-1 and  LRH-1 binding to the PE1, PE2, and DR0 probes in the absence or presence of antibodies.	bind
81475	3	3764	11	NULL	NULL	0	NULL	SF-1	GeneOrProtein	COS1-overexpressed	binds to 					PE2 probe	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_9_3492_s_146	15831456	(B) COS1-overexpressed SF-1 and  LRH-1 binding to the PE1, PE2, and DR0 probes in the absence or presence of antibodies.	bind
81476	4	3764	11	NULL	NULL	0	NULL	 LRH-1	GeneOrProtein	COS1-overexpressed	binds to 					PE2 probe	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_9_3492_s_146	15831456	(B) COS1-overexpressed SF-1 and  LRH-1 binding to the PE1, PE2, and DR0 probes in the absence or presence of antibodies.	bind
81477	5	3764	11	NULL	NULL	0	NULL	SF-1	GeneOrProtein	COS1-overexpressed	binds to 					DR0 probe	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_9_3492_s_146	15831456	(B) COS1-overexpressed SF-1 and  LRH-1 binding to the PE1, PE2, and DR0 probes in the absence or presence of antibodies.	bind
81478	6	3764	11	NULL	NULL	0	NULL	LRH-1	GeneOrProtein	COS1-overexpressed	binds to 					DR0 probe	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_9_3492_s_146	15831456	(B) COS1-overexpressed SF-1 and  LRH-1 binding to the PE1, PE2, and DR0 probes in the absence or presence of antibodies.	bind
8688	1	3765	5	11	NULL	NULL	NULL	HIF-1	GP		bind					f-actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_273_2_285_s_73	15328013	(B) Costaining for HIF-1  (green) and phalloidin-Alexa Fluor 568 (red),  which binds f-actin and delineates the myocardium.	bind
8689	2	3765	5	11	NULL	NULL	NULL	HIF-1	GP		delineates					myocardium	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_273_2_285_s_73	15328013	(B) Costaining for HIF-1  (green) and phalloidin-Alexa Fluor 568 (red),  which binds f-actin and delineates the myocardium.	bind
8690	3	3765	5	11	NULL	NULL	NULL	phalloidin-Alexa Fluor 568	Chemical		bind					f-actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_273_2_285_s_73	15328013	(B) Costaining for HIF-1  (green) and phalloidin-Alexa Fluor 568 (red),  which binds f-actin and delineates the myocardium.	bind
8691	4	3765	5	11	NULL	NULL	NULL	phalloidin-Alexa Fluor 568	Chemical		delineates					myocardium	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_273_2_285_s_73	15328013	(B) Costaining for HIF-1  (green) and phalloidin-Alexa Fluor 568 (red),  which binds f-actin and delineates the myocardium.	bind
9053	1	3765	6	11	NULL	NULL	NULL	HIF-1	GP		bind					F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_273_2_285_s_73	15328013	(B) Costaining for HIF-1  (green) and phalloidin-Alexa Fluor 568 (red),  which binds f-actin and delineates the myocardium.	bind
9054	2	3765	6	11	NULL	NULL	NULL	phalloidin-Alexa Fluor 568	Chemical		bind					F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_273_2_285_s_73	15328013	(B) Costaining for HIF-1  (green) and phalloidin-Alexa Fluor 568 (red),  which binds f-actin and delineates the myocardium.	bind
9055	3	3765	6	11	NULL	NULL	NULL	statement 1	Process		delineates					myocardium	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_273_2_285_s_73	15328013	(B) Costaining for HIF-1  (green) and phalloidin-Alexa Fluor 568 (red),  which binds f-actin and delineates the myocardium.	bind
9056	4	3765	6	11	NULL	NULL	NULL	statement 2	Process		delineates					myocardium	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_273_2_285_s_73	15328013	(B) Costaining for HIF-1  (green) and phalloidin-Alexa Fluor 568 (red),  which binds f-actin and delineates the myocardium.	bind
81479	1	3765	11	NULL	NULL	NULL	NULL	phalloidin-Alexa Fluor 568	NonProteinOrNucleicAcidChemical		binds to 					f-actin	GeneOrProtein				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_273_2_285_s_73	15328013	(B) Costaining for HIF-1  (green) and phalloidin-Alexa Fluor 568 (red),  which binds f-actin and delineates the myocardium.	bind
81480	2	3765	11	NULL	NULL	0	NULL	statement 1	Process		delineates					myocardium	AnatomicalPart				NULL		0	NULL	NULL	NULL	gw70_devbiol_273_2_285_s_73	15328013	(B) Costaining for HIF-1  (green) and phalloidin-Alexa Fluor 568 (red),  which binds f-actin and delineates the myocardium.	bind
8692	1	3766	5	11	NULL	NULL	NULL	BV	Chemical		bind		covalently			PHY-2	GP		1-515		NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_4_12_2140_s_190	16339731	(B) Covalent binding of BV and  PCB to PHY-2 (1-515).	bind
8693	2	3766	5	11	NULL	NULL	NULL	PCB	GP		bind		covalently			PHY-2	GP		1-515		NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_4_12_2140_s_190	16339731	(B) Covalent binding of BV and  PCB to PHY-2 (1-515).	bind
9057	1	3766	6	11	NULL	NULL	NULL	BV	Chemical		bind		covalently			PHY-2	GP		1-515		NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_4_12_2140_s_190	16339731	(B) Covalent binding of BV and  PCB to PHY-2 (1-515).	bind
9058	2	3766	6	11	NULL	NULL	NULL	PCB	GP		bind		covalently			PHY-2	GP		1-515		NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_4_12_2140_s_190	16339731	(B) Covalent binding of BV and  PCB to PHY-2 (1-515).	bind
81481	1	3766	11	NULL	NULL	0	NULL	BV	Chemical		binds to 		Covalently			PHY-2	Protein				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_12_2140_s_190	16339731	(B) Covalent binding of BV and  PCB to PHY-2 (1-515).	bind
81482	2	3766	11	NULL	NULL	0	NULL	PCB	Chemical		binds to 		Covalently			PHY-2	Protein				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_12_2140_s_190	16339731	(B) Covalent binding of BV and  PCB to PHY-2 (1-515).	bind
8694	1	3767	5	11	NULL	NULL	NULL	CP110	GP		bind					cyclin E/CDK2	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_devcell_3_3_339_s_69	12361598	(B) CP110 binds to cyclin E/CDK2, cyclin A/CDK2, and cyclin B/CDC2 in vitro.	bind
8695	2	3767	5	11	NULL	NULL	NULL	CP110	GP		bind					cyclin A/CDK2	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_devcell_3_3_339_s_69	12361598	(B) CP110 binds to cyclin E/CDK2, cyclin A/CDK2, and cyclin B/CDC2 in vitro.	bind
8696	3	3767	5	11	NULL	NULL	NULL	CP110	GP		bind					cyclin B/CDC2	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_devcell_3_3_339_s_69	12361598	(B) CP110 binds to cyclin E/CDK2, cyclin A/CDK2, and cyclin B/CDC2 in vitro.	bind
9059	1	3767	6	11	NULL	NULL	NULL	CP110	GP		bind					cyclin E/CDK2	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_devcell_3_3_339_s_69	12361598	(B) CP110 binds to cyclin E/CDK2, cyclin A/CDK2, and cyclin B/CDC2 in vitro.	bind
9060	2	3767	6	11	NULL	NULL	NULL	CP110	GP		bind					cyclin A/CDK2	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_devcell_3_3_339_s_69	12361598	(B) CP110 binds to cyclin E/CDK2, cyclin A/CDK2, and cyclin B/CDC2 in vitro.	bind
9061	3	3767	6	11	NULL	NULL	NULL	CP110	GP		bind					cyclin B/CDC2	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_devcell_3_3_339_s_69	12361598	(B) CP110 binds to cyclin E/CDK2, cyclin A/CDK2, and cyclin B/CDC2 in vitro.	bind
81483	1	3767	11	NULL	NULL	0	NULL	CP110	GeneOrProtein		binds to 					cyclin E/CDK2	GeneOrProtein				NULL	in vitro	0	NULL	NULL	NULL	gw60_devcell_3_3_339_s_69	12361598	(B) CP110 binds to cyclin E/CDK2, cyclin A/CDK2, and cyclin B/CDC2 in vitro.	bind
81484	2	3767	11	NULL	NULL	0	NULL	CP110	GeneOrProtein		binds to 					 cyclin A/CDK2	GeneOrProtein				NULL	in vitro	0	NULL	NULL	NULL	gw60_devcell_3_3_339_s_69	12361598	(B) CP110 binds to cyclin E/CDK2, cyclin A/CDK2, and cyclin B/CDC2 in vitro.	bind
81485	3	3767	11	NULL	NULL	0	NULL	CP110	GeneOrProtein		binds to 					 cyclin B/CDC2	GeneOrProtein				NULL	in vitro	0	NULL	NULL	NULL	gw60_devcell_3_3_339_s_69	12361598	(B) CP110 binds to cyclin E/CDK2, cyclin A/CDK2, and cyclin B/CDC2 in vitro.	bind
8697	1	3768	5	11	NULL	NULL	NULL	CR	GP		bind					TRAF2	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_5_409_s_73	11882293	(B) CR binds TRAF2 through the N-terminal non-death domain region.	bind
8698	2	3768	5	11	NULL	NULL	NULL	statement 1	Process		occurs through								N-terminal non-death domain region		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_5_409_s_73	11882293	(B) CR binds TRAF2 through the N-terminal non-death domain region.	bind
9062	1	3768	6	11	NULL	NULL	NULL	CR	GP		bind			N-terminal non-death domain region		TRAF2	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_5_409_s_73	11882293	(B) CR binds TRAF2 through the N-terminal non-death domain region.	bind
81486	1	3768	11	NULL	NULL	0	NULL	crinkled	GeneOrProtein		binds to 			N-terminal non-death domain		TRAF2	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_currbiol_12_5_409_s_73	11882293	(B) CR binds TRAF2 through the N-terminal non-death domain region.	bind
8699	1	3769	5	11	NULL	NULL	NULL	CREB1a 	GP		forms					homo-dimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_95_2_211_s_98	9790528	(B) CREB1a and CREB1b bind CRE as homo- and heterodimers.	bind
8700	2	3769	5	11	NULL	NULL	NULL	CREB1b	GP		forms					homo-dimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_95_2_211_s_98	9790528	(B) CREB1a and CREB1b bind CRE as homo- and heterodimers.	bind
8701	3	3769	5	11	NULL	NULL	NULL	CREB1a	GP		forms					heterodimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_95_2_211_s_98	9790528	(B) CREB1a and CREB1b bind CRE as homo- and heterodimers.	bind
8702	5	3769	5	11	NULL	NULL	NULL	statement 1	GP		bind									CRE	NULL		NULL	NULL	NULL	NULL	gw60_cell_95_2_211_s_98	9790528	(B) CREB1a and CREB1b bind CRE as homo- and heterodimers.	bind
11088	4	3769	5	11	NULL	NULL	NULL	CREB1b	GP		forms					heterodimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_95_2_211_s_98	9790528	(B) CREB1a and CREB1b bind CRE as homo- and heterodimers.	bind
53479	6	3769	5	11	NULL	NULL	NULL	statement 2	GP		bind									CRE	NULL		NULL	NULL	NULL	NULL	gw60_cell_95_2_211_s_98	9790528	(B) CREB1a and CREB1b bind CRE as homo- and heterodimers.	bind
53480	7	3769	5	11	NULL	NULL	NULL	statement 3	GP		bind									CRE	NULL		NULL	NULL	NULL	NULL	gw60_cell_95_2_211_s_98	9790528	(B) CREB1a and CREB1b bind CRE as homo- and heterodimers.	bind
53481	8	3769	5	11	NULL	NULL	NULL	statement 4	GP		bind									CRE	NULL		NULL	NULL	NULL	NULL	gw60_cell_95_2_211_s_98	9790528	(B) CREB1a and CREB1b bind CRE as homo- and heterodimers.	bind
9063	1	3769	6	11	NULL	NULL	NULL	CREB1a	GP		form					homodimers	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_95_2_211_s_98	9790528	(B) CREB1a and CREB1b bind CRE as homo- and heterodimers.	bind
9064	2	3769	6	11	NULL	NULL	NULL	statement 1	GP		bind									CRE	NULL		NULL	NULL	NULL	NULL	gw60_cell_95_2_211_s_98	9790528	(B) CREB1a and CREB1b bind CRE as homo- and heterodimers.	bind
9358	3	3769	6	11	NULL	NULL	NULL	CREB1b	GP		form					homodimers	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_95_2_211_s_98	9790528	(B) CREB1a and CREB1b bind CRE as homo- and heterodimers.	bind
9359	5	3769	6	11	NULL	NULL	NULL	CREB1a	GP		forms					heterodimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_95_2_211_s_98	9790528	(B) CREB1a and CREB1b bind CRE as homo- and heterodimers.	bind
9360	6	3769	6	11	NULL	NULL	NULL	CREB1b	GP		forms					heterodimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_95_2_211_s_98	9790528	(B) CREB1a and CREB1b bind CRE as homo- and heterodimers.	bind
9362	4	3769	6	11	NULL	NULL	NULL	statement 3	GP		bind									CRE	NULL		NULL	NULL	NULL	NULL	gw60_cell_95_2_211_s_98	9790528	(B) CREB1a and CREB1b bind CRE as homo- and heterodimers.	bind
9363	7	3769	6	11	NULL	NULL	NULL	statement 5	GP		bind									CRE	NULL		NULL	NULL	NULL	NULL	gw60_cell_95_2_211_s_98	9790528	(B) CREB1a and CREB1b bind CRE as homo- and heterodimers.	bind
53482	8	3769	6	11	NULL	NULL	NULL	statement 6	GP		bind									CRE	NULL		NULL	NULL	NULL	NULL	gw60_cell_95_2_211_s_98	9790528	(B) CREB1a and CREB1b bind CRE as homo- and heterodimers.	bind
81487	1	3769	11	NULL	NULL	0	NULL	CREB1a	GeneOrProtein		binds to 					CRE	Gene				NULL		0	NULL	NULL	NULL	gw60_cell_95_2_211_s_98	9790528	(B) CREB1a and CREB1b bind CRE as homo- and heterodimers.	bind
81488	2	3769	11	NULL	NULL	0	NULL	CREB1b	GeneOrProtein		binds to 					CRE	Gene				NULL		0	NULL	NULL	NULL	gw60_cell_95_2_211_s_98	9790528	(B) CREB1a and CREB1b bind CRE as homo- and heterodimers.	bind
8872	1	3770	5	11	NULL	NULL	NULL	DBP	GP	purified;;serum	bind					cell surface	OrganismPart				NULL	wild-type kidneys	NULL	NULL	NULL	NULL	gw60_cell_96_4_507_s_91	10052453	(B) Cryosections  through wild-type and megalin-/- kidneys were incubated with purified serum DBP, and cell  surface binding of DBP was detected using rabbit anti-DBP antiserum and peroxidase-conjugated  anti-rabbit IgG.	bind
53634	2	3770	5	11	NULL	NULL	NULL	DBP	GP	purified;;serum	bind					cell surface	OrganismPart				NULL	megalin-/- kidneys	NULL	NULL	NULL	NULL	gw60_cell_96_4_507_s_91	10052453	(B) Cryosections  through wild-type and megalin-/- kidneys were incubated with purified serum DBP, and cell  surface binding of DBP was detected using rabbit anti-DBP antiserum and peroxidase-conjugated  anti-rabbit IgG.	bind
9065	1	3770	6	11	NULL	NULL	NULL	DBP	GP	purified;;serum	bind					cell surface	OrganismPart				NULL	wild type kidneys	NULL	NULL	NULL	NULL	gw60_cell_96_4_507_s_91	10052453	(B) Cryosections  through wild-type and megalin-/- kidneys were incubated with purified serum DBP, and cell  surface binding of DBP was detected using rabbit anti-DBP antiserum and peroxidase-conjugated  anti-rabbit IgG.	bind
9066	2	3770	6	11	NULL	NULL	NULL	DBP	GP	purified;;serum	bind					cell surface	OrganismPart				NULL	megalin-/- kidneys	NULL	NULL	NULL	NULL	gw60_cell_96_4_507_s_91	10052453	(B) Cryosections  through wild-type and megalin-/- kidneys were incubated with purified serum DBP, and cell  surface binding of DBP was detected using rabbit anti-DBP antiserum and peroxidase-conjugated  anti-rabbit IgG.	bind
81489	1	3770	11	NULL	NULL	0	NULL	DBP	Protein	serum 	binds to 					cell surface	CellComponent				NULL		0	NULL	NULL	NULL	gw60_cell_96_4_507_s_91	10052453	(B) Cryosections  through wild-type and megalin-/- kidneys were incubated with purified serum DBP, and cell  surface binding of DBP was detected using rabbit anti-DBP antiserum and peroxidase-conjugated  anti-rabbit IgG.	bind
8703	1	3771	5	11	NULL	NULL	NULL	CSC-1	GP		bind					BIR-1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_cellbiol_161_2_229_s_106	12707312	(B) CSC-1 binds to BIR-1 in vitro, and this interaction requires Zinc binding  by BIR-1.	bind
8704	2	3771	5	11	NULL	NULL	NULL	BIR-1	GP		bind					Zinc	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_161_2_229_s_106	12707312	(B) CSC-1 binds to BIR-1 in vitro, and this interaction requires Zinc binding  by BIR-1.	bind
8705	3	3771	5	11	NULL	NULL	NULL	statement 1	Process		require					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_161_2_229_s_106	12707312	(B) CSC-1 binds to BIR-1 in vitro, and this interaction requires Zinc binding  by BIR-1.	bind
9067	1	3771	6	11	NULL	NULL	NULL	Zinc	Chemical		bind					BIR-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_161_2_229_s_106	12707312	(B) CSC-1 binds to BIR-1 in vitro, and this interaction requires Zinc binding  by BIR-1.	bind
9068	2	3771	6	11	NULL	NULL	NULL	BIR-1	GP		bind					CSC-1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_cellbiol_161_2_229_s_106	12707312	(B) CSC-1 binds to BIR-1 in vitro, and this interaction requires Zinc binding  by BIR-1.	bind
9700	3	3771	6	11	NULL	NULL	NULL	statement 2	Process		require					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_161_2_229_s_106	12707312	(B) CSC-1 binds to BIR-1 in vitro, and this interaction requires Zinc binding  by BIR-1.	bind
81490	1	3771	11	NULL	NULL	0	NULL	CSC-1	GeneOrProtein		binds to 					BIR-1	GeneOrProtein				NULL	in vitro	0	NULL	NULL	NULL	gw70_cellbiol_161_2_229_s_106	12707312	(B) CSC-1 binds to BIR-1 in vitro, and this interaction requires Zinc binding  by BIR-1.	bind
81491	2	3771	11	NULL	NULL	0	NULL	Zinc	NonProteinOrNucleicAcidChemical		binds to 					BIR-1	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw70_cellbiol_161_2_229_s_106	12707312	(B) CSC-1 binds to BIR-1 in vitro, and this interaction requires Zinc binding  by BIR-1.	bind
81492	3	3771	11	NULL	NULL	0	NULL	statement 2	Process		requires					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_cellbiol_161_2_229_s_106	12707312	(B) CSC-1 binds to BIR-1 in vitro, and this interaction requires Zinc binding  by BIR-1.	bind
8706	1	3773	5	11	NULL	NULL	NULL	CtBP2	GP		bind					Znf219	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_15_5296_s_284	12101226	(B) CtBP2 binds Znf219 in vitro.	bind
9069	1	3773	6	11	NULL	NULL	NULL	CtBP2	GP		bind					Znf219	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_15_5296_s_284	12101226	(B) CtBP2 binds Znf219 in vitro.	bind
81493	1	3773	11	NULL	NULL	0	NULL	CtBP2	GeneOrProtein		binds to 					Znf219	GeneOrProtein				NULL	in vitro	0	NULL	NULL	NULL	gw60_molcellbiol_22_15_5296_s_284	12101226	(B) CtBP2 binds Znf219 in vitro.	bind
8712	1	3774	5	11	NULL	NULL	NULL	CUG-BP	GP		bind									U/G motifs in 3 splice site of intron 2	NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_1_45_s_148	12150906	(B) CUG-BP binds U/G motifs in the 3  splice site of intron 2.	bind
9070	1	3774	6	11	NULL	NULL	NULL	CUG-BP	GP		bind									U/G motifs in 3 splice site of intron 2	NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_1_45_s_148	12150906	(B) CUG-BP binds U/G motifs in the 3  splice site of intron 2.	bind
81494	1	3774	11	NULL	NULL	0	NULL	CUG-BP	GeneOrProtein		binds to 					intron 2	NucleicAcidSubstance			U/G motifs	NULL		0	NULL	NULL	NULL	gw60_molcell_10_1_45_s_148	12150906	(B) CUG-BP binds U/G motifs in the 3  splice site of intron 2.	bind
8713	1	3775	5	11	NULL	NULL	NULL	BCE	GP		bind					Hb	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_8_2528_s_169	12670977	(b) Curve for the binding of BCE surface  proteins to Hb after neutralization of Hb binding.	bind
53635	2	3775	5	11	NULL	NULL	NULL	BCE	GP		is a type of					surface protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_8_2528_s_169	12670977	(b) Curve for the binding of BCE surface  proteins to Hb after neutralization of Hb binding.	bind
9071	1	3775	6	11	NULL	NULL	NULL	BCE 	GP		bind					Hb	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_8_2528_s_169	12670977	(b) Curve for the binding of BCE surface  proteins to Hb after neutralization of Hb binding.	bind
41005	2	3775	6	11	NULL	NULL	NULL	BCE	GP		is a type of					surface protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_8_2528_s_169	12670977	(b) Curve for the binding of BCE surface  proteins to Hb after neutralization of Hb binding.	bind
81495	1	3775	11	NULL	NULL	0	NULL	BCE surface protein	Protein		binds to 					Hb	CellComponent				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_8_2528_s_169	12670977	(b) Curve for the binding of BCE surface  proteins to Hb after neutralization of Hb binding.	bind
8714	1	3776	5	11	NULL	NULL	NULL	AgrA	GP		bind							isolated		P2 repeats	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_22_7549_s_157	15516566	(B) Curves showing binding  of AgrA to isolated P2 and P3 repeats and to a P2 mutant fragment.	bind
8715	2	3776	5	11	NULL	NULL	NULL	AgrA	GP		bind							isolated		P3 repeats	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_22_7549_s_157	15516566	(B) Curves showing binding  of AgrA to isolated P2 and P3 repeats and to a P2 mutant fragment.	bind
8716	3	3776	5	11	NULL	NULL	NULL	AgrA	GP		bind							mutant		P2 fragment	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_22_7549_s_157	15516566	(B) Curves showing binding  of AgrA to isolated P2 and P3 repeats and to a P2 mutant fragment.	bind
9072	1	3776	6	11	NULL	NULL	NULL	AgrA	GP		bind							isolated		P2 repeats	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_22_7549_s_157	15516566	(B) Curves showing binding  of AgrA to isolated P2 and P3 repeats and to a P2 mutant fragment.	bind
9073	2	3776	6	11	NULL	NULL	NULL	AgrA	GP		bind							isolated		P3 repeats	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_22_7549_s_157	15516566	(B) Curves showing binding  of AgrA to isolated P2 and P3 repeats and to a P2 mutant fragment.	bind
9074	3	3776	6	11	NULL	NULL	NULL	AgrA	GP		bind							mutant		P2 fragment	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_22_7549_s_157	15516566	(B) Curves showing binding  of AgrA to isolated P2 and P3 repeats and to a P2 mutant fragment.	bind
81503	1	3776	11	NULL	NULL	0	NULL	AgrA	GeneOrProtein		binds to 					P2 repeat	Gene				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_22_7549_s_157	15516566	(B) Curves showing binding  of AgrA to isolated P2 and P3 repeats and to a P2 mutant fragment.	bind
81504	2	3776	11	NULL	NULL	0	NULL	AgrA	GeneOrProtein		binds to 					P3 repeat	Gene				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_22_7549_s_157	15516566	(B) Curves showing binding  of AgrA to isolated P2 and P3 repeats and to a P2 mutant fragment.	bind
81506	3	3776	11	NULL	NULL	0	NULL	AgrA	GeneOrProtein		binds to 					P2 fragment	Gene	mutant			NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_22_7549_s_157	15516566	(B) Curves showing binding  of AgrA to isolated P2 and P3 repeats and to a P2 mutant fragment.	bind
8717	1	3777	5	11	NULL	NULL	NULL	p130 constructs	GP	transfected	bind					Cyclin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5380_s_269	9710622	(B) Cyclin-binding activity of transfected p130 constructs.	bind
9075	1	3777	6	11	NULL	NULL	NULL	p130 constructs	GP	transfected	bind					Cyclin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5380_s_269	9710622	(B) Cyclin-binding activity of transfected p130 constructs.	bind
81507	1	3777	11	NULL	NULL	0	NULL	Cyclin	GeneOrProtein		binds to 					p130	GeneOrProtein	transfected			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_9_5380_s_269	9710622	(B) Cyclin-binding activity of transfected p130 constructs.	bind
8718	1	3778	5	11	NULL	NULL	NULL	Cyp-40	GP		bind					c-Myb	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_203_s_102	9659917	(B) Cyclosporin-A does not affect Cyp-40 binding to c-Myb.	bind
8719	2	3778	5	11	NULL	NULL	NULL	Cyclosporin-A	Chemical		does not affect					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_203_s_102	9659917	(B) Cyclosporin-A does not affect Cyp-40 binding to c-Myb.	bind
9076	1	3778	6	11	NULL	NULL	NULL	Cyp-40	GP		bind					c-Myb	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_203_s_102	9659917	(B) Cyclosporin-A does not affect Cyp-40 binding to c-Myb.	bind
9077	2	3778	6	11	NULL	NULL	NULL	Cyclosporin-A	Chemical		does not affect					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_2_203_s_102	9659917	(B) Cyclosporin-A does not affect Cyp-40 binding to c-Myb.	bind
81508	1	3778	11	NULL	NULL	0	NULL	Cyp-40	GeneOrProtein		binds to 					c-Myb	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_molcell_1_2_203_s_102	9659917	(B) Cyclosporin-A does not affect Cyp-40 binding to c-Myb.	bind
81509	2	3778	11	NULL	NULL	0	NULL	Cyclosporin-A	Chemical		does not affect					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_1_2_203_s_102	9659917	(B) Cyclosporin-A does not affect Cyp-40 binding to c-Myb.	bind
8720	1	3779	5	11	NULL	NULL	NULL	Dap1p	GP		bind					heme	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1669_s_139	15713626	(B) Dap1p bound to heme (left bar), while the Dap1pD91G lost heme-binding activity (right bar).	bind
8721	2	3779	5	11	NULL	NULL	NULL	Dap1p	GP		does not bind			D91G		heme	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1669_s_139	15713626	(B) Dap1p bound to heme (left bar), while the Dap1pD91G lost heme-binding activity (right bar).	bind
9078	1	3779	6	11	NULL	NULL	NULL	Dap1p	GP		bind					heme	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1669_s_139	15713626	(B) Dap1p bound to heme (left bar), while the Dap1pD91G lost heme-binding activity (right bar).	bind
9079	2	3779	6	11	NULL	NULL	NULL	Dap1p	GP		does not bind			D91G		heme	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1669_s_139	15713626	(B) Dap1p bound to heme (left bar), while the Dap1pD91G lost heme-binding activity (right bar).	bind
81510	1	3779	11	NULL	NULL	0	NULL	Dap1p	Protein		binds to 					heme	Protein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_5_1669_s_139	15713626	(B) Dap1p bound to heme (left bar), while the Dap1pD91G lost heme-binding activity (right bar).	bind
8722	1	3780	5	11	NULL	NULL	NULL	DAPA	Chemical		bind					DTBS	GP				NULL		NULL	NULL	NULL	NULL	gw60_structure_3_11_1207_s_85	8591031	(b) DAPA bound to DTBS, in 20 mM MgSO4 and in a CO2-free nitrogen atmosphere.	bind
8723	2	3780	5	11	NULL	NULL	NULL	statement 1	Process		occurs in					MgSO4	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_structure_3_11_1207_s_85	8591031	(b) DAPA bound to DTBS, in 20 mM MgSO4 and in a CO2-free nitrogen atmosphere.	bind
8724	3	3780	5	11	NULL	NULL	NULL	statement 1	Process		occurs in					CO2-free nitrogen atmosphere	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_structure_3_11_1207_s_85	8591031	(b) DAPA bound to DTBS, in 20 mM MgSO4 and in a CO2-free nitrogen atmosphere.	bind
9080	1	3780	6	11	NULL	NULL	NULL	DAPA	Chemical		bind					DTBS	GP				NULL		NULL	NULL	NULL	NULL	gw60_structure_3_11_1207_s_85	8591031	(b) DAPA bound to DTBS, in 20 mM MgSO4 and in a CO2-free nitrogen atmosphere.	bind
9081	2	3780	6	11	NULL	NULL	NULL	statement 1	Process		occurs in					CO2-free nitrogen atmosphere	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_structure_3_11_1207_s_85	8591031	(b) DAPA bound to DTBS, in 20 mM MgSO4 and in a CO2-free nitrogen atmosphere.	bind
9082	3	3780	6	11	NULL	NULL	NULL	statement 1	Process		occurs in					MgSO4	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_structure_3_11_1207_s_85	8591031	(b) DAPA bound to DTBS, in 20 mM MgSO4 and in a CO2-free nitrogen atmosphere.	bind
81512	1	3780	11	NULL	NULL	0	NULL	DAPA	NonProteinOrNucleicAcidChemical		binds to 					DTBS	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_structure_3_11_1207_s_85	8591031	(b) DAPA bound to DTBS, in 20 mM MgSO4 and in a CO2-free nitrogen atmosphere.	bind
81513	2	3780	11	NULL	NULL	0	NULL	statement 1	Process		occurs in the presence of					MgSO4	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	gw60_structure_3_11_1207_s_85	8591031	(b) DAPA bound to DTBS, in 20 mM MgSO4 and in a CO2-free nitrogen atmosphere.	bind
81514	3	3780	11	NULL	NULL	0	NULL	statement 1	Process		occurs in the presence of					CO2-free nitrogen	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	gw60_structure_3_11_1207_s_85	8591031	(b) DAPA bound to DTBS, in 20 mM MgSO4 and in a CO2-free nitrogen atmosphere.	bind
8725	1	3782	5	11	NULL	NULL	NULL	Daxx	GP		bind					p53	GP		COOH terminus		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_1_322_s_120	12482984	(B) Daxx binds to the COOH terminus of p53.	bind
9083	1	3782	6	11	NULL	NULL	NULL	Daxx	GP		bind					p53	GP		COOH terminus		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_1_322_s_120	12482984	(B) Daxx binds to the COOH terminus of p53.	bind
81515	1	3782	11	NULL	NULL	0	NULL	Daxx	GeneOrProtein		binds to 					p53	Protein		COOH terminus		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_1_322_s_120	12482984	(B) Daxx binds to the COOH terminus of p53.	bind
8726	1	3783	5	NULL	NULL	0	NULL	Daxx	NULL		bind	NULL				p53	NULL	mutants			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_1_322_s_166	12482984	(B) Daxx binds to various p53 mutants.	bind
9084	1	3783	6	NULL	NULL	0	NULL	Daxx	NULL		bind	NULL				p53	NULL	mutant			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_1_322_s_166	12482984	(B) Daxx binds to various p53 mutants.	bind
81516	1	3783	11	NULL	NULL	0	NULL	Daxx	GeneOrProtein		binds to 					p53	Gene	mutant			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_1_322_s_166	12482984	(B) Daxx binds to various p53 mutants.	bind
8727	1	3784	5	11	NULL	NULL	NULL	Ddi1	GP		bind			UBL domain		19S RP	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5355_s_131	15964793	(B) Ddi1 binds the 19S RP via its UBL domain.	bind
9085	1	3784	6	11	NULL	NULL	NULL	Ddi1	GP		bind			UBL domain		19S RP	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5355_s_131	15964793	(B) Ddi1 binds the 19S RP via its UBL domain.	bind
81517	1	3784	11	NULL	NULL	0	NULL	Ddi1	PartOfProtein		binds to 					19S RP	Protein		UBL domain		NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_13_5355_s_131	15964793	(B) Ddi1 binds the 19S RP via its UBL domain.	bind
8728	1	3785	5	11	NULL	NULL	NULL	ZO-1	GP		bind					GST-C-Occludin(NP)	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_67	12604349	(B) Densitometric  analysis of ZO-1, ZO-2, and ZO-3 bound to GST-C-Occludin(NP) and GST-C-Occludin(PY)  in A. Values (arbitrary density units) are average of three independent experiments.	bind
8729	2	3785	5	11	NULL	NULL	NULL	ZO-2	GP		bind					GST-C-Occludin(NP)	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_67	12604349	(B) Densitometric  analysis of ZO-1, ZO-2, and ZO-3 bound to GST-C-Occludin(NP) and GST-C-Occludin(PY)  in A. Values (arbitrary density units) are average of three independent experiments.	bind
8730	3	3785	5	11	NULL	NULL	NULL	ZO-3	GP		bind					GST-C-Occludin(NP)	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_67	12604349	(B) Densitometric  analysis of ZO-1, ZO-2, and ZO-3 bound to GST-C-Occludin(NP) and GST-C-Occludin(PY)  in A. Values (arbitrary density units) are average of three independent experiments.	bind
8731	4	3785	5	11	NULL	NULL	NULL	ZO-1	GP		bind					GST-C-Occludin(PY)	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_67	12604349	(B) Densitometric  analysis of ZO-1, ZO-2, and ZO-3 bound to GST-C-Occludin(NP) and GST-C-Occludin(PY)  in A. Values (arbitrary density units) are average of three independent experiments.	bind
8732	5	3785	5	11	NULL	NULL	NULL	ZO-2	GP		bind					GST-C-Occludin(PY)	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_67	12604349	(B) Densitometric  analysis of ZO-1, ZO-2, and ZO-3 bound to GST-C-Occludin(NP) and GST-C-Occludin(PY)  in A. Values (arbitrary density units) are average of three independent experiments.	bind
8733	6	3785	5	11	NULL	NULL	NULL	ZO-3	GP		bind					GST-C-Occludin(PY)	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_67	12604349	(B) Densitometric  analysis of ZO-1, ZO-2, and ZO-3 bound to GST-C-Occludin(NP) and GST-C-Occludin(PY)  in A. Values (arbitrary density units) are average of three independent experiments.	bind
9086	1	3785	6	11	NULL	NULL	NULL	ZO-1	GP		bind					GST-C-Occludin(NP)	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_67	12604349	(B) Densitometric  analysis of ZO-1, ZO-2, and ZO-3 bound to GST-C-Occludin(NP) and GST-C-Occludin(PY)  in A. Values (arbitrary density units) are average of three independent experiments.	bind
9087	2	3785	6	11	NULL	NULL	NULL	ZO-1	GP		bind					GST-C-Occludin(PY)	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_67	12604349	(B) Densitometric  analysis of ZO-1, ZO-2, and ZO-3 bound to GST-C-Occludin(NP) and GST-C-Occludin(PY)  in A. Values (arbitrary density units) are average of three independent experiments.	bind
9088	3	3785	6	11	NULL	NULL	NULL	ZO-2	GP		bind					GST-C-Occludin(NP)	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_67	12604349	(B) Densitometric  analysis of ZO-1, ZO-2, and ZO-3 bound to GST-C-Occludin(NP) and GST-C-Occludin(PY)  in A. Values (arbitrary density units) are average of three independent experiments.	bind
9089	4	3785	6	11	NULL	NULL	NULL	ZO-2	GP		bind					GST-C-Occludin(PY)	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_67	12604349	(B) Densitometric  analysis of ZO-1, ZO-2, and ZO-3 bound to GST-C-Occludin(NP) and GST-C-Occludin(PY)  in A. Values (arbitrary density units) are average of three independent experiments.	bind
9090	5	3785	6	11	NULL	NULL	NULL	ZO-3	GP		bind					GST-C-Occludin(NP)	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_67	12604349	(B) Densitometric  analysis of ZO-1, ZO-2, and ZO-3 bound to GST-C-Occludin(NP) and GST-C-Occludin(PY)  in A. Values (arbitrary density units) are average of three independent experiments.	bind
9091	6	3785	6	11	NULL	NULL	NULL	ZO-3	GP		bind					GST-C-Occludin(PY)	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_67	12604349	(B) Densitometric  analysis of ZO-1, ZO-2, and ZO-3 bound to GST-C-Occludin(NP) and GST-C-Occludin(PY)  in A. Values (arbitrary density units) are average of three independent experiments.	bind
81518	1	3785	11	NULL	NULL	0	NULL	GST-C-Occludin	Protein		is					NP	Protein				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_67	12604349	(B) Densitometric  analysis of ZO-1, ZO-2, and ZO-3 bound to GST-C-Occludin(NP) and GST-C-Occludin(PY)  in A. Values (arbitrary density units) are average of three independent experiments.	bind
81519	2	3785	11	NULL	NULL	0	NULL	GST-C-Occludin	Protein		binds to 					PY	Protein				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_67	12604349	(B) Densitometric  analysis of ZO-1, ZO-2, and ZO-3 bound to GST-C-Occludin(NP) and GST-C-Occludin(PY)  in A. Values (arbitrary density units) are average of three independent experiments.	bind
81521	3	3785	11	NULL	NULL	NULL	NULL	ZO-1	Protein		binds to 					GST-C-Occludin	Protein				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_67	12604349	(B) Densitometric  analysis of ZO-1, ZO-2, and ZO-3 bound to GST-C-Occludin(NP) and GST-C-Occludin(PY)  in A. Values (arbitrary density units) are average of three independent experiments.	bind
81522	4	3785	11	NULL	NULL	0	NULL	ZO-1	Protein		binds to 					GST-C-Occludin	Protein				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_67	12604349	(B) Densitometric  analysis of ZO-1, ZO-2, and ZO-3 bound to GST-C-Occludin(NP) and GST-C-Occludin(PY)  in A. Values (arbitrary density units) are average of three independent experiments.	bind
81523	5	3785	11	NULL	NULL	0	NULL	ZO-2	Protein		binds to 					GST-C-Occludin	Protein				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_67	12604349	(B) Densitometric  analysis of ZO-1, ZO-2, and ZO-3 bound to GST-C-Occludin(NP) and GST-C-Occludin(PY)  in A. Values (arbitrary density units) are average of three independent experiments.	bind
81524	6	3785	11	NULL	NULL	0	NULL	ZO-2	Protein		binds to 					GST-C-Occludin	Protein				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_67	12604349	(B) Densitometric  analysis of ZO-1, ZO-2, and ZO-3 bound to GST-C-Occludin(NP) and GST-C-Occludin(PY)  in A. Values (arbitrary density units) are average of three independent experiments.	bind
81525	7	3785	11	NULL	NULL	0	NULL	ZO-3	Protein		binds to 					GST-C-Occludin	Protein				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_67	12604349	(B) Densitometric  analysis of ZO-1, ZO-2, and ZO-3 bound to GST-C-Occludin(NP) and GST-C-Occludin(PY)  in A. Values (arbitrary density units) are average of three independent experiments.	bind
81526	8	3785	11	NULL	NULL	0	NULL	ZO-3	Protein		binds to 					GST-C-Occludin	Protein				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_67	12604349	(B) Densitometric  analysis of ZO-1, ZO-2, and ZO-3 bound to GST-C-Occludin(NP) and GST-C-Occludin(PY)  in A. Values (arbitrary density units) are average of three independent experiments.	bind
8734	1	3787	5	11	NULL	NULL	NULL	ZO-1	GP		bind					GST-C-Occludin(NP)	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_79	12604349	(B) Densitometric analysis of ZO-1, ZO-2, and ZO-3  bound to GST-C-Occludin(NP) and GST-C-Occludin(PY) in A. Values (arbitrary density  units) are average of values from two independent experiments.	bind
8735	2	3787	5	11	NULL	NULL	NULL	ZO-2	GP		bind					GST-C-Occludin(NP)	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_79	12604349	(B) Densitometric analysis of ZO-1, ZO-2, and ZO-3  bound to GST-C-Occludin(NP) and GST-C-Occludin(PY) in A. Values (arbitrary density  units) are average of values from two independent experiments.	bind
8736	3	3787	5	11	NULL	NULL	NULL	ZO-3	GP		bind					GST-C-Occludin(NP)	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_79	12604349	(B) Densitometric analysis of ZO-1, ZO-2, and ZO-3  bound to GST-C-Occludin(NP) and GST-C-Occludin(PY) in A. Values (arbitrary density  units) are average of values from two independent experiments.	bind
8737	4	3787	5	11	NULL	NULL	NULL	ZO-1	GP		bind					GST-C-Occludin(PY)	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_79	12604349	(B) Densitometric analysis of ZO-1, ZO-2, and ZO-3  bound to GST-C-Occludin(NP) and GST-C-Occludin(PY) in A. Values (arbitrary density  units) are average of values from two independent experiments.	bind
8738	5	3787	5	11	NULL	NULL	NULL	ZO-2	GP		bind					GST-C-Occludin(PY)	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_79	12604349	(B) Densitometric analysis of ZO-1, ZO-2, and ZO-3  bound to GST-C-Occludin(NP) and GST-C-Occludin(PY) in A. Values (arbitrary density  units) are average of values from two independent experiments.	bind
8739	6	3787	5	11	NULL	NULL	NULL	ZO-3	GP		bind					GST-C-Occludin(PY)	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_79	12604349	(B) Densitometric analysis of ZO-1, ZO-2, and ZO-3  bound to GST-C-Occludin(NP) and GST-C-Occludin(PY) in A. Values (arbitrary density  units) are average of values from two independent experiments.	bind
9092	1	3787	6	11	NULL	NULL	NULL	ZO-1	GP		bind					GST-C-Occludin(NP)	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_79	12604349	(B) Densitometric analysis of ZO-1, ZO-2, and ZO-3  bound to GST-C-Occludin(NP) and GST-C-Occludin(PY) in A. Values (arbitrary density  units) are average of values from two independent experiments.	bind
9093	2	3787	6	11	NULL	NULL	NULL	ZO-1	GP		bind					GST-C-Occludin(PY)	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_79	12604349	(B) Densitometric analysis of ZO-1, ZO-2, and ZO-3  bound to GST-C-Occludin(NP) and GST-C-Occludin(PY) in A. Values (arbitrary density  units) are average of values from two independent experiments.	bind
9094	3	3787	6	11	NULL	NULL	NULL	ZO-2	GP		bind					GST-C-Occludin(NP)	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_79	12604349	(B) Densitometric analysis of ZO-1, ZO-2, and ZO-3  bound to GST-C-Occludin(NP) and GST-C-Occludin(PY) in A. Values (arbitrary density  units) are average of values from two independent experiments.	bind
9095	4	3787	6	11	NULL	NULL	NULL	ZO-2	GP		bind					GST-C-Occludin(PY)	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_79	12604349	(B) Densitometric analysis of ZO-1, ZO-2, and ZO-3  bound to GST-C-Occludin(NP) and GST-C-Occludin(PY) in A. Values (arbitrary density  units) are average of values from two independent experiments.	bind
9096	5	3787	6	11	NULL	NULL	NULL	ZO-3	GP		bind					GST-C-Occludin(NP)	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_79	12604349	(B) Densitometric analysis of ZO-1, ZO-2, and ZO-3  bound to GST-C-Occludin(NP) and GST-C-Occludin(PY) in A. Values (arbitrary density  units) are average of values from two independent experiments.	bind
9097	6	3787	6	11	NULL	NULL	NULL	ZO-3	GP		bind					GST-C-Occludin(PY)	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_2_324_s_79	12604349	(B) Densitometric analysis of ZO-1, ZO-2, and ZO-3  bound to GST-C-Occludin(NP) and GST-C-Occludin(PY) in A. Values (arbitrary density  units) are average of values from two independent experiments.	bind
9098	1	3788	6	11	NULL	NULL	NULL	ZO-1	GP		bind					GST-C-Occludin(NP)	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_302_2_324_s_67	12604349	(B) Densitometric analysis of ZO-1, ZO-2, and ZO-3 bound to GST-C-Occludin(NP) and GST-C-Occludin(PY) in A. Values (arbitrary density units) are average of three independent experiments.	bind
9099	2	3788	6	11	NULL	NULL	NULL	ZO-1	GP		bind					GST-C-Occludin(PY)	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_302_2_324_s_67	12604349	(B) Densitometric analysis of ZO-1, ZO-2, and ZO-3 bound to GST-C-Occludin(NP) and GST-C-Occludin(PY) in A. Values (arbitrary density units) are average of three independent experiments.	bind
9100	3	3788	6	11	NULL	NULL	NULL	ZO-2	GP		bind					GST-C-Occludin(NP)	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_302_2_324_s_67	12604349	(B) Densitometric analysis of ZO-1, ZO-2, and ZO-3 bound to GST-C-Occludin(NP) and GST-C-Occludin(PY) in A. Values (arbitrary density units) are average of three independent experiments.	bind
9101	4	3788	6	11	NULL	NULL	NULL	ZO-2	GP		bind					GST-C-Occludin(PY)	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_302_2_324_s_67	12604349	(B) Densitometric analysis of ZO-1, ZO-2, and ZO-3 bound to GST-C-Occludin(NP) and GST-C-Occludin(PY) in A. Values (arbitrary density units) are average of three independent experiments.	bind
9102	5	3788	6	11	NULL	NULL	NULL	ZO-3	GP		bind					GST-C-Occludin(NP)	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_302_2_324_s_67	12604349	(B) Densitometric analysis of ZO-1, ZO-2, and ZO-3 bound to GST-C-Occludin(NP) and GST-C-Occludin(PY) in A. Values (arbitrary density units) are average of three independent experiments.	bind
9103	6	3788	6	11	NULL	NULL	NULL	ZO-3	GP		bind					GST-C-Occludin(PY)	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_302_2_324_s_67	12604349	(B) Densitometric analysis of ZO-1, ZO-2, and ZO-3 bound to GST-C-Occludin(NP) and GST-C-Occludin(PY) in A. Values (arbitrary density units) are average of three independent experiments.	bind
8746	1	3790	5	11	NULL	NULL	NULL	TcTS	GP		interact with					lactose	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_4_757_s_147	12419220	(b) Detailed view of the interaction between TcTS and lactose, demonstrating that the acceptor substrate only binds to TcTS when sialic acid is present.	bind
8747	2	3790	5	11	NULL	NULL	NULL	acceptor substrate	Chemical		bind					TcTS	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_4_757_s_147	12419220	(b) Detailed view of the interaction between TcTS and lactose, demonstrating that the acceptor substrate only binds to TcTS when sialic acid is present.	bind
8748	3	3790	5	11	NULL	NULL	NULL	statement 2	Process		in the presence of		only			sialic acid	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_4_757_s_147	12419220	(b) Detailed view of the interaction between TcTS and lactose, demonstrating that the acceptor substrate only binds to TcTS when sialic acid is present.	bind
9104	1	3790	6	11	NULL	NULL	NULL	TcTS	GP		interacts with					lactose	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_4_757_s_147	12419220	(b) Detailed view of the interaction between TcTS and lactose, demonstrating that the acceptor substrate only binds to TcTS when sialic acid is present.	bind
9105	2	3790	6	11	NULL	NULL	NULL	acceptor substrate	Chemical		bind					TcTS	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_4_757_s_147	12419220	(b) Detailed view of the interaction between TcTS and lactose, demonstrating that the acceptor substrate only binds to TcTS when sialic acid is present.	bind
9106	3	3790	6	11	NULL	NULL	NULL	statement 2	Process		occurs in presence of		only			sialic acid	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_4_757_s_147	12419220	(b) Detailed view of the interaction between TcTS and lactose, demonstrating that the acceptor substrate only binds to TcTS when sialic acid is present.	bind
81529	1	3790	11	NULL	NULL	0	NULL	TcTS	GeneOrProtein		interacts with					lactose	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	gw60_molcell_10_4_757_s_147	12419220	(b) Detailed view of the interaction between TcTS and lactose, demonstrating that the acceptor substrate only binds to TcTS when sialic acid is present.	bind
81530	2	3790	11	NULL	NULL	0	NULL	acceptor substrate	Thing		binds to 					TcTS	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_molcell_10_4_757_s_147	12419220	(b) Detailed view of the interaction between TcTS and lactose, demonstrating that the acceptor substrate only binds to TcTS when sialic acid is present.	bind
81531	3	3790	11	NULL	NULL	0	NULL	statement 2	Process		occurs in the presence of					sialic acid	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	gw60_molcell_10_4_757_s_147	12419220	(b) Detailed view of the interaction between TcTS and lactose, demonstrating that the acceptor substrate only binds to TcTS when sialic acid is present.	bind
8749	1	3791	5	11	NULL	NULL	NULL	ras	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_4282_s_212	9632812	(B) Detection of an active, GTP-bound form of ras during treatment with rhTPO or rhIL-3.	bind
9174	1	3791	6	11	NULL	NULL	NULL	GTP	Chemical		bind					ras	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_4282_s_212	9632812	(B) Detection of an active, GTP-bound form of ras during treatment with rhTPO or rhIL-3.	bind
81532	1	3791	11	NULL	NULL	0	NULL	GTP	NonProteinOrNucleicAcidChemical		binds to 					ras	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_7_4282_s_212	9632812	(B) Detection of an active, GTP-bound form of ras during treatment with rhTPO or rhIL-3.	bind
8750	1	3794	5	11	NULL	NULL	NULL	RCH1	GP		bind					CAS	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_11_7782_s_161	10523667	(B) Determination of the binding affinities of importin alpha1/Rch1 (RCH1), importin alpha5/hSRP1 (hSRP1), and importin alpha3 to CAS.	bind
8751	2	3794	5	11	NULL	NULL	NULL	RCH1	GP		is					importin alpha1/Rch1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_11_7782_s_161	10523667	(B) Determination of the binding affinities of importin alpha1/Rch1 (RCH1), importin alpha5/hSRP1 (hSRP1), and importin alpha3 to CAS.	bind
8752	3	3794	5	11	NULL	NULL	NULL	hSRP1	GP		bind					CAS	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_11_7782_s_161	10523667	(B) Determination of the binding affinities of importin alpha1/Rch1 (RCH1), importin alpha5/hSRP1 (hSRP1), and importin alpha3 to CAS.	bind
8753	4	3794	5	11	NULL	NULL	NULL	hSRP1	GP		is					importin alpha5/hSRP1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_11_7782_s_161	10523667	(B) Determination of the binding affinities of importin alpha1/Rch1 (RCH1), importin alpha5/hSRP1 (hSRP1), and importin alpha3 to CAS.	bind
8754	5	3794	5	11	NULL	NULL	NULL	importin alpha3	GP		bind					CAS	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_11_7782_s_161	10523667	(B) Determination of the binding affinities of importin alpha1/Rch1 (RCH1), importin alpha5/hSRP1 (hSRP1), and importin alpha3 to CAS.	bind
9175	1	3794	6	11	NULL	NULL	NULL	importin alpha1/Rch1	GP		bind					CAS	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_11_7782_s_161	10523667	(B) Determination of the binding affinities of importin alpha1/Rch1 (RCH1), importin alpha5/hSRP1 (hSRP1), and importin alpha3 to CAS.	bind
9176	2	3794	6	11	NULL	NULL	NULL	importin alpha5/hSRP1	GP		bind					CAS	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_11_7782_s_161	10523667	(B) Determination of the binding affinities of importin alpha1/Rch1 (RCH1), importin alpha5/hSRP1 (hSRP1), and importin alpha3 to CAS.	bind
9177	3	3794	6	11	NULL	NULL	NULL	importin alpha3	GP		bind					CAS	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_11_7782_s_161	10523667	(B) Determination of the binding affinities of importin alpha1/Rch1 (RCH1), importin alpha5/hSRP1 (hSRP1), and importin alpha3 to CAS.	bind
11649	4	3794	6	11	NULL	NULL	NULL	RCH1	GP		is					importin alpha1/Rch1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_11_7782_s_161	10523667	(B) Determination of the binding affinities of importin alpha1/Rch1 (RCH1), importin alpha5/hSRP1 (hSRP1), and importin alpha3 to CAS.	bind
11650	5	3794	6	11	NULL	NULL	NULL	hSRP1	GP		is					importin alpha5/hSRP1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_11_7782_s_161	10523667	(B) Determination of the binding affinities of importin alpha1/Rch1 (RCH1), importin alpha5/hSRP1 (hSRP1), and importin alpha3 to CAS.	bind
81533	1	3794	11	NULL	NULL	0	NULL	importin alpha1/Rch1	Protein		is					RCH1	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_11_7782_s_161	10523667	(B) Determination of the binding affinities of importin alpha1/Rch1 (RCH1), importin alpha5/hSRP1 (hSRP1), and importin alpha3 to CAS.	bind
81534	2	3794	11	NULL	NULL	0	NULL	importin alpha5/hSRP1	Protein		binds to 					hSRP1	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_11_7782_s_161	10523667	(B) Determination of the binding affinities of importin alpha1/Rch1 (RCH1), importin alpha5/hSRP1 (hSRP1), and importin alpha3 to CAS.	bind
81535	3	3794	11	NULL	NULL	0	NULL	importin alpha1/Rch1	GeneOrProtein		binds to 					CAS	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_11_7782_s_161	10523667	(B) Determination of the binding affinities of importin alpha1/Rch1 (RCH1), importin alpha5/hSRP1 (hSRP1), and importin alpha3 to CAS.	bind
81536	4	3794	11	NULL	NULL	0	NULL	importin alpha5/hSRP1	GeneOrProtein		binds to 					CAS	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_11_7782_s_161	10523667	(B) Determination of the binding affinities of importin alpha1/Rch1 (RCH1), importin alpha5/hSRP1 (hSRP1), and importin alpha3 to CAS.	bind
81537	5	3794	11	NULL	NULL	0	NULL	importin alpha3	GeneOrProtein		binds to 					CAS	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_11_7782_s_161	10523667	(B) Determination of the binding affinities of importin alpha1/Rch1 (RCH1), importin alpha5/hSRP1 (hSRP1), and importin alpha3 to CAS.	bind
8755	1	3795	5	11	NULL	NULL	NULL	dHK protein	GP		bind					microtubules	CellComponent	endogenous;; Drosophila			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_923_s_240	11238449	(B) dHK protein also bound to endogenous  Drosophila microtubules when they were stabilized by the addition of GTP - taxol.	bind
8756	2	3795	5	11	NULL	NULL	NULL	GTP - taxol	Chemical	addition of	stabilize					microtubules	CellComponent	endogenous;;Drosophila			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_923_s_240	11238449	(B) dHK protein also bound to endogenous  Drosophila microtubules when they were stabilized by the addition of GTP - taxol.	bind
8757	3	3795	5	11	NULL	NULL	NULL	statement 1	Process		occurs after					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_923_s_240	11238449	(B) dHK protein also bound to endogenous  Drosophila microtubules when they were stabilized by the addition of GTP - taxol.	bind
9178	1	3795	6	11	NULL	NULL	NULL	dHK protein	GP		bind					microtubules	CellComponent	endogenous;; Drosophila			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_923_s_240	11238449	(B) dHK protein also bound to endogenous  Drosophila microtubules when they were stabilized by the addition of GTP - taxol.	bind
9179	2	3795	6	11	NULL	NULL	NULL	GTP-taxol	Chemical		stabilizes					microtubules	CellComponent	endogenous;; drosophila			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_923_s_240	11238449	(B) dHK protein also bound to endogenous  Drosophila microtubules when they were stabilized by the addition of GTP - taxol.	bind
9180	3	3795	6	11	NULL	NULL	NULL	statement 2	Process		leads to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_923_s_240	11238449	(B) dHK protein also bound to endogenous  Drosophila microtubules when they were stabilized by the addition of GTP - taxol.	bind
81538	1	3795	11	NULL	NULL	NULL	NULL	GTP - taxol	NonProteinOrNucleicAcidChemical		stabilizes 					endogenous microtubules	CellComponent	Drosophila			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_923_s_240	11238449	(B) dHK protein also bound to endogenous  Drosophila microtubules when they were stabilized by the addition of GTP - taxol.	bind
81539	2	3795	11	NULL	NULL	0	NULL	dHK protein	Protein		binds to 					endogenous microtubules\t\t\t 	CellComponent	Drosophila			NULL		0	NULL	NULL	NULL	gw60_cellbiol_152_5_923_s_240	11238449	(B) dHK protein also bound to endogenous  Drosophila microtubules when they were stabilized by the addition of GTP - taxol.	bind
81540	3	3795	11	NULL	NULL	0	NULL	statement 2	Process		occurs after					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_152_5_923_s_240	11238449	(B) dHK protein also bound to endogenous  Drosophila microtubules when they were stabilized by the addition of GTP - taxol.	bind
8903	1	3796	5	11	NULL	NULL	NULL	preimmune serum	CellComponent	rabbit	bind					Dap.3	Cell				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_6_2769_s_108	10338479	(B) Dilution studies of antisera raised against CKDLL EQKRAAVDTYC, CLGSIS ESRRALQDSQR, and CKDIL EDERAAVDTYC peptides and pooled preimmune rabbit serum binding to mouse fibroblast transfected cell line Dap.3 expressing HLA-DRB1*0401 (DR4/Dw4).	bind
8904	2	3796	5	11	NULL	NULL	NULL	Dap.3	cell		is a type of					 fibroblast transfected cell line 	Cell	mouse			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_6_2769_s_108	10338479	(B) Dilution studies of antisera raised against CKDLL EQKRAAVDTYC, CLGSIS ESRRALQDSQR, and CKDIL EDERAAVDTYC peptides and pooled preimmune rabbit serum binding to mouse fibroblast transfected cell line Dap.3 expressing HLA-DRB1*0401 (DR4/Dw4).	bind
53641	3	3796	5	11	NULL	NULL	NULL	Dap.3	cell		express					HLA-DRB1*0401 (DR4/Dw4)	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_6_2769_s_108	10338479	(B) Dilution studies of antisera raised against CKDLL EQKRAAVDTYC, CLGSIS ESRRALQDSQR, and CKDIL EDERAAVDTYC peptides and pooled preimmune rabbit serum binding to mouse fibroblast transfected cell line Dap.3 expressing HLA-DRB1*0401 (DR4/Dw4).	bind
9181	1	3796	6	11	NULL	NULL	NULL	Dap.3	cell		expresses					HLA-DRB1*0401 (DR4/Dw4)	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_6_2769_s_108	10338479	(B) Dilution studies of antisera raised against CKDLL EQKRAAVDTYC, CLGSIS ESRRALQDSQR, and CKDIL EDERAAVDTYC peptides and pooled preimmune rabbit serum binding to mouse fibroblast transfected cell line Dap.3 expressing HLA-DRB1*0401 (DR4/Dw4).	bind
9182	2	3796	6	11	NULL	NULL	NULL	preimmune serum	CellComponent	 rabbit	bind					Dap.3	Cell				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_6_2769_s_108	10338479	(B) Dilution studies of antisera raised against CKDLL EQKRAAVDTYC, CLGSIS ESRRALQDSQR, and CKDIL EDERAAVDTYC peptides and pooled preimmune rabbit serum binding to mouse fibroblast transfected cell line Dap.3 expressing HLA-DRB1*0401 (DR4/Dw4).	bind
41006	3	3796	6	11	NULL	NULL	NULL	Dap.3	cell		is a type of					fibroblast transfected cell line	Cell	mouse			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_6_2769_s_108	10338479	(B) Dilution studies of antisera raised against CKDLL EQKRAAVDTYC, CLGSIS ESRRALQDSQR, and CKDIL EDERAAVDTYC peptides and pooled preimmune rabbit serum binding to mouse fibroblast transfected cell line Dap.3 expressing HLA-DRB1*0401 (DR4/Dw4).	bind
81541	1	3796	11	NULL	NULL	NULL	NULL	preimmune serum	CellComponent	rabbit	binds to 					statement 3	Cell				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_6_2769_s_108	10338479	(B) Dilution studies of antisera raised against CKDLL EQKRAAVDTYC, CLGSIS ESRRALQDSQR, and CKDIL EDERAAVDTYC peptides and pooled preimmune rabbit serum binding to mouse fibroblast transfected cell line Dap.3 expressing HLA-DRB1*0401 (DR4/Dw4).	bind
81542	2	3796	11	NULL	NULL	0	NULL	fibroblast cell\t	cell	mouse	is					Dap.3	Cell				NULL		0	NULL	NULL	NULL	gw60_infectimmun_67_6_2769_s_108	10338479	(B) Dilution studies of antisera raised against CKDLL EQKRAAVDTYC, CLGSIS ESRRALQDSQR, and CKDIL EDERAAVDTYC peptides and pooled preimmune rabbit serum binding to mouse fibroblast transfected cell line Dap.3 expressing HLA-DRB1*0401 (DR4/Dw4).	bind
81543	3	3796	11	NULL	NULL	0	NULL	Dap.3	cell		express					HLA-DRB1	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_infectimmun_67_6_2769_s_108	10338479	(B) Dilution studies of antisera raised against CKDLL EQKRAAVDTYC, CLGSIS ESRRALQDSQR, and CKDIL EDERAAVDTYC peptides and pooled preimmune rabbit serum binding to mouse fibroblast transfected cell line Dap.3 expressing HLA-DRB1*0401 (DR4/Dw4).	bind
81544	4	3796	11	NULL	NULL	0	NULL	peptides	PartOfProtein		binds to 			CKDLL EQKRAAVDTYC		statement 3	Cell				NULL		0	NULL	NULL	NULL	gw60_infectimmun_67_6_2769_s_108	10338479	(B) Dilution studies of antisera raised against CKDLL EQKRAAVDTYC, CLGSIS ESRRALQDSQR, and CKDIL EDERAAVDTYC peptides and pooled preimmune rabbit serum binding to mouse fibroblast transfected cell line Dap.3 expressing HLA-DRB1*0401 (DR4/Dw4).	bind
81545	5	3796	11	NULL	NULL	0	NULL	peptides	PartOfProtein		binds to 			CLGSIS ESRRALQDSQR		statement 3	Cell				NULL		0	NULL	NULL	NULL	gw60_infectimmun_67_6_2769_s_108	10338479	(B) Dilution studies of antisera raised against CKDLL EQKRAAVDTYC, CLGSIS ESRRALQDSQR, and CKDIL EDERAAVDTYC peptides and pooled preimmune rabbit serum binding to mouse fibroblast transfected cell line Dap.3 expressing HLA-DRB1*0401 (DR4/Dw4).	bind
81546	6	3796	11	NULL	NULL	0	NULL	peptides	PartOfProtein		binds to 			CKDIL EDERAAVDTYC		statement 3	Cell				NULL		0	NULL	NULL	NULL	gw60_infectimmun_67_6_2769_s_108	10338479	(B) Dilution studies of antisera raised against CKDLL EQKRAAVDTYC, CLGSIS ESRRALQDSQR, and CKDIL EDERAAVDTYC peptides and pooled preimmune rabbit serum binding to mouse fibroblast transfected cell line Dap.3 expressing HLA-DRB1*0401 (DR4/Dw4).	bind
8905	1	3797	5	11	NULL	NULL	NULL	calmodulin	GP		bind		directly			L-selectin	GP		cytoplasmic tail		NULL		NULL	NULL	NULL	NULL	gw60_cell_92_6_809_s_104	9529256	(B) Direct binding of calmodulin to  the L-selectin cytoplasmic tail.	bind
9183	1	3797	6	11	NULL	NULL	NULL	calmodulin	GP		bind		directly			L-selectin	GP		cytoplasmic tail		NULL		NULL	NULL	NULL	NULL	gw60_cell_92_6_809_s_104	9529256	(B) Direct binding of calmodulin to  the L-selectin cytoplasmic tail.	bind
81547	1	3797	11	NULL	NULL	0	NULL	calmodulin	GeneOrProtein		binds to 		direct			L-selectin	Protein		cytoplasmic tail		NULL		0	NULL	NULL	NULL	gw60_cell_92_6_809_s_104	9529256	(B) Direct binding of calmodulin to  the L-selectin cytoplasmic tail.	bind
8906	1	3798	5	11	NULL	NULL	NULL	Dam1	GP		bind		directly			Ipl1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_5_763_s_139	11724818	(B) Direct binding of Dam1 to Ipl1 and Sli15.	bind
8907	2	3798	5	11	NULL	NULL	NULL	Dam1	GP		bind		directly			Sli15	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_5_763_s_139	11724818	(B) Direct binding of Dam1 to Ipl1 and Sli15.	bind
9184	1	3798	6	11	NULL	NULL	NULL	Dam1	GP		bind		directly			Ipl1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_5_763_s_139	11724818	(B) Direct binding of Dam1 to Ipl1 and Sli15.	bind
9185	2	3798	6	11	NULL	NULL	NULL	Dam1	GP		bind		directly			Sli15	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_5_763_s_139	11724818	(B) Direct binding of Dam1 to Ipl1 and Sli15.	bind
81548	1	3798	11	NULL	NULL	0	NULL	Dam1	GeneOrProtein		binds to 		direct			Ipl1	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_cellbiol_155_5_763_s_139	11724818	(B) Direct binding of Dam1 to Ipl1 and Sli15.	bind
81549	2	3798	11	NULL	NULL	0	NULL	Dam1	GeneOrProtein		binds to 		direct			Sli15	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_cellbiol_155_5_763_s_139	11724818	(B) Direct binding of Dam1 to Ipl1 and Sli15.	bind
8908	1	3799	5	11	NULL	NULL	NULL	alphaCP-1	GP	recombinant	bind		directly							alpha3'UTR	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4572_s_219	10373506	(B) Direct binding of recombinant alphaCP-1 and alphaCP-2 to the alpha3'UTR (determined as detailed for panel A).	bind
8909	2	3799	5	11	NULL	NULL	NULL	alphaCP-2	GP	recombinant	bind		directly							alpha3'UTR	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4572_s_219	10373506	(B) Direct binding of recombinant alphaCP-1 and alphaCP-2 to the alpha3'UTR (determined as detailed for panel A).	bind
53642	3	3799	5	11	NULL	NULL	NULL	alphaCP-1	GP		is a type of					recombinant protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4572_s_219	10373506	(B) Direct binding of recombinant alphaCP-1 and alphaCP-2 to the alpha3'UTR (determined as detailed for panel A).	bind
53644	4	3799	5	11	NULL	NULL	NULL	alphaCP-2	GP		is a type of					recombinant protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4572_s_219	10373506	(B) Direct binding of recombinant alphaCP-1 and alphaCP-2 to the alpha3'UTR (determined as detailed for panel A).	bind
9186	1	3799	6	11	NULL	NULL	NULL	alphaCP-1	GP		bind		directly							alpha3'UTR	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4572_s_219	10373506	(B) Direct binding of recombinant alphaCP-1 and alphaCP-2 to the alpha3'UTR (determined as detailed for panel A).	bind
9187	2	3799	6	11	NULL	NULL	NULL	alphaCP-2	GP		bind		directly							alpha3'UTR	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4572_s_219	10373506	(B) Direct binding of recombinant alphaCP-1 and alphaCP-2 to the alpha3'UTR (determined as detailed for panel A).	bind
41007	3	3799	6	11	NULL	NULL	NULL	alphaCP-1	GP		is a type of					recombinant protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4572_s_219	10373506	(B) Direct binding of recombinant alphaCP-1 and alphaCP-2 to the alpha3'UTR (determined as detailed for panel A).	bind
41008	4	3799	6	11	NULL	NULL	NULL	alphaCP-2	GP		is a type of					recombinant protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4572_s_219	10373506	(B) Direct binding of recombinant alphaCP-1 and alphaCP-2 to the alpha3'UTR (determined as detailed for panel A).	bind
81550	1	3799	11	NULL	NULL	0	NULL	alphaCP-1	GeneOrProtein	recombinant	binds to 		direct			alpha3'UTR	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_7_4572_s_219	10373506	(B) Direct binding of recombinant alphaCP-1 and alphaCP-2 to the alpha3'UTR (determined as detailed for panel A).	bind
81551	2	3799	11	NULL	NULL	0	NULL	alphaCP-2	GeneOrProtein	recombinant	binds to 		direct			alpha3'UTR	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_7_4572_s_219	10373506	(B) Direct binding of recombinant alphaCP-1 and alphaCP-2 to the alpha3'UTR (determined as detailed for panel A).	bind
8910	1	3800	5	11	NULL	NULL	NULL	RIM1	GP		bind		directly			CAST	GP		COOH terminus		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_158_3_577_s_208	12163476	(b) Direct binding of RIM1 to the COOH terminus of CAST.	bind
9188	1	3800	6	11	NULL	NULL	NULL	RIM1	GP		bind		directly			CAST	GP		COOH terminus		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_158_3_577_s_208	12163476	(b) Direct binding of RIM1 to the COOH terminus of CAST.	bind
81552	1	3800	11	NULL	NULL	0	NULL	RIM1	GeneOrProtein		binds to 					CAST	Protein		COOH terminus		NULL		0	NULL	NULL	NULL	gw60_cellbiol_158_3_577_s_208	12163476	(b) Direct binding of RIM1 to the COOH terminus of CAST.	bind
8911	1	3801	5	11	NULL	NULL	NULL	tomosyn	GP		bind		directly			syntaxin-1a	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_20_5_905_s_79	9620695	(B) Direct binding of tomosyn to syntaxin-1a in a blot overlay assay.	bind
9189	1	3801	6	11	NULL	NULL	NULL	tomosyn	GP		bind		directly			syntaxin 1a	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_20_5_905_s_79	9620695	(B) Direct binding of tomosyn to syntaxin-1a in a blot overlay assay.	bind
81553	1	3801	11	NULL	NULL	0	NULL	tomosyn	GeneOrProtein		binds to 		direct			syntaxin-1a	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_neuron_20_5_905_s_79	9620695	(B) Direct binding of tomosyn to syntaxin-1a in a blot overlay assay.	bind
8912	1	3802	5	11	NULL	NULL	NULL	SHP-1	GP		bind					CD22	GP	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_18_1009_s_191	9740800	(b) Distinction between function of SHP-1 bound to tyrosine-phosphorylated CD22 and CD72, respectively.	bind
8913	2	3802	5	11	NULL	NULL	NULL	SHP-1	GP		bind					CD72	GP	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_18_1009_s_191	9740800	(b) Distinction between function of SHP-1 bound to tyrosine-phosphorylated CD22 and CD72, respectively.	bind
9190	1	3802	6	11	NULL	NULL	NULL	SHP-1	GP		bind					CD22	GP	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_18_1009_s_191	9740800	(b) Distinction between function of SHP-1 bound to tyrosine-phosphorylated CD22 and CD72, respectively.	bind
9191	2	3802	6	11	NULL	NULL	NULL	SHP-1	GP		bind					CD72	GP	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_18_1009_s_191	9740800	(b) Distinction between function of SHP-1 bound to tyrosine-phosphorylated CD22 and CD72, respectively.	bind
81554	1	3802	11	NULL	NULL	0	NULL	SHP-1	GeneOrProtein		binds to 					CD22	Protein		tyrosine-phosphorylated 		NULL		0	NULL	NULL	NULL	gw60_currbiol_8_18_1009_s_191	9740800	(b) Distinction between function of SHP-1 bound to tyrosine-phosphorylated CD22 and CD72, respectively.	bind
81555	2	3802	11	NULL	NULL	0	NULL	SHP-1	GeneOrProtein		binds to 					CD72	Protein		tyrosine-phosphorylated		NULL		0	NULL	NULL	NULL	gw60_currbiol_8_18_1009_s_191	9740800	(b) Distinction between function of SHP-1 bound to tyrosine-phosphorylated CD22 and CD72, respectively.	bind
8914	1	3804	5	11	NULL	NULL	NULL	p53 protein	GP	endogenous	bind									p53BE	NULL		NULL	NULL	NULL	NULL	gw60_cell_113_3_301_s_279	12732139	(B) DNAP showing Activin-independent binding of endogenous p53 protein to  p53BE.	bind
8915	2	3804	5	11	NULL	NULL	NULL	statement 1	Process		is independent of					activin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_113_3_301_s_279	12732139	(B) DNAP showing Activin-independent binding of endogenous p53 protein to  p53BE.	bind
9192	1	3804	6	11	NULL	NULL	NULL	p53 protein	GP	endogenous	bind									p53BE	NULL		NULL	NULL	NULL	NULL	gw60_cell_113_3_301_s_279	12732139	(B) DNAP showing Activin-independent binding of endogenous p53 protein to  p53BE.	bind
9193	2	3804	6	11	NULL	NULL	NULL	statement 1	Process		is independent of					activin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_113_3_301_s_279	12732139	(B) DNAP showing Activin-independent binding of endogenous p53 protein to  p53BE.	bind
81556	1	3804	11	NULL	NULL	NULL	NULL	p53 protein	Protein	 endogenous	binds to 					p53BE	Gene				NULL		NULL	NULL	NULL	NULL	gw60_cell_113_3_301_s_279	12732139	(B) DNAP showing Activin-independent binding of endogenous p53 protein to  p53BE.	bind
81557	2	3804	11	NULL	NULL	0	NULL	statement 1	Process		is independent of					statement 3	Protein				NULL		0	NULL	NULL	NULL	gw60_cell_113_3_301_s_279	12732139	(B) DNAP showing Activin-independent binding of endogenous p53 protein to  p53BE.	bind
81558	3	3804	11	NULL	NULL	0	NULL	DNAP	GeneOrProtein		shows					Activin	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_cell_113_3_301_s_279	12732139	(B) DNAP showing Activin-independent binding of endogenous p53 protein to  p53BE.	bind
8916	1	3805	5	11	NULL	NULL	NULL	NAC	GP		bind					gdhA	GP			promoter region	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_24_6966_s_100	12446647	(B) DNase I footprint of NAC bound to the  gdhA promoter region.	bind
9194	1	3805	6	11	NULL	NULL	NULL	NAC	GP		bind					gdhA	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_24_6966_s_100	12446647	(B) DNase I footprint of NAC bound to the  gdhA promoter region.	bind
81559	1	3805	11	NULL	NULL	0	NULL	NAC	GeneOrProtein		binds to 				DNase I footprint	 gdhA	Gene			promoter region	NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_24_6966_s_100	12446647	(B) DNase I footprint of NAC bound to the  gdhA promoter region.	bind
8917	1	3807	5	11	NULL	NULL	NULL	Zur	GP		bind					yciA	GP			promoter region	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_23_6508_s_153	12426338	(B) DNase I footprinting analysis of Zur binding to the  yciA promoter region.	bind
9195	1	3807	6	11	NULL	NULL	NULL	Zur	GP		bind					yciA	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_23_6508_s_153	12426338	(B) DNase I footprinting analysis of Zur binding to the  yciA promoter region.	bind
81560	1	3807	11	NULL	NULL	0	NULL	Zur	GeneOrProtein		binds to 				DNase I footprinting	 yciA	Gene			promoter region	NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_23_6508_s_153	12426338	(B) DNase I footprinting analysis of Zur binding to the  yciA promoter region.	bind
8918	1	3808	5	11	NULL	NULL	NULL	YycF	GP		bind					ssaA	GP			promoter region	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_4_1175_s_151	14762013	(B) DNase I footprinting of YycF bound to the  ssaA promoter region.	bind
9196	1	3808	6	11	NULL	NULL	NULL	YycF	GP		bind					ssaA	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_4_1175_s_151	14762013	(B) DNase I footprinting of YycF bound to the  ssaA promoter region.	bind
81561	1	3808	11	NULL	NULL	0	NULL	YycF	GeneOrProtein		binds to 				DNase I footprint	ssaA	Gene			promoter region	NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_4_1175_s_151	14762013	(B) DNase I footprinting of YycF bound to the  ssaA promoter region.	bind
8919	1	3809	5	11	NULL	NULL	NULL	Doa1	GP		bind					Ub	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4122_s_134	16705165	(B) Doa1  binds Ub in vitro.	bind
9197	1	3809	6	11	NULL	NULL	NULL	Doa1	GP		bind					Ub	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4122_s_134	16705165	(B) Doa1  binds Ub in vitro.	bind
81562	1	3809	11	NULL	NULL	0	NULL	Doa1	GeneOrProtein		binds to 					Ub	GeneOrProtein				NULL	in vitro	0	NULL	NULL	NULL	gw70_molcellbiol_26_11_4122_s_134	16705165	(B) Doa1  binds Ub in vitro.	bind
8920	1	3810	5	11	NULL	NULL	NULL	DOKL	GP		bind					c-Abl	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8314_s_276	10567556	(B) DOKL binding to c-Abl requires Abl kinase activity.	bind
8921	2	3810	5	11	NULL	NULL	NULL	statement 1	Process		require					Abl kinase	GP	 activity of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8314_s_276	10567556	(B) DOKL binding to c-Abl requires Abl kinase activity.	bind
9198	1	3810	6	11	NULL	NULL	NULL	DOKL	GP		bind					c-Abl	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8314_s_276	10567556	(B) DOKL binding to c-Abl requires Abl kinase activity.	bind
41009	3	3810	6	11	NULL	NULL	NULL	statement 1	Process		requires					Abl kinase	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8314_s_276	10567556	(B) DOKL binding to c-Abl requires Abl kinase activity.	bind
81563	1	3810	11	NULL	NULL	0	NULL	DOKL	GeneOrProtein		binds to 					c-Abl	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_12_8314_s_276	10567556	(B) DOKL binding to c-Abl requires Abl kinase activity.	bind
81564	2	3810	11	NULL	NULL	0	NULL	statement 1	Process		requires					Abl kinase	Protein				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_12_8314_s_276	10567556	(B) DOKL binding to c-Abl requires Abl kinase activity.	bind
8922	1	3811	5	11	NULL	NULL	NULL				bind		dose dependently	LR974P		SHP-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1545_1_20_s_143	11342028	(B) Dose dependence of binding of LR974P to SHP-2.	bind
9200	1	3811	6	11	NULL	NULL	NULL				bind		dose dependently	LR974P		SHP-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1545_1_20_s_143	11342028	(B) Dose dependence of binding of LR974P to SHP-2.	bind
81600	1	3811	11	NULL	NULL	0	NULL	LR974P	GeneOrProtein		binds to 					SHP2	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1545_1_20_s_143	11342028	(B) Dose dependence of binding of LR974P to SHP-2.	bind
8924	1	3812	5	11	NULL	NULL	NULL	Raf-1	GP		bind					GST-Rb	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_137	15485920	(B) Dose-dependent inhibition of the binding of  Raf-1 to GST-Rb by the Raf-1 peptide in a GST pull-down assay.	bind
8925	2	3812	5	11	NULL	NULL	NULL	Raf-1 peptide	GP		inhibits		dose-dependently			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_137	15485920	(B) Dose-dependent inhibition of the binding of  Raf-1 to GST-Rb by the Raf-1 peptide in a GST pull-down assay.	bind
9201	1	3812	6	11	NULL	NULL	NULL	Raf-1	GP		bind					GST-Rb	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_137	15485920	(B) Dose-dependent inhibition of the binding of  Raf-1 to GST-Rb by the Raf-1 peptide in a GST pull-down assay.	bind
9202	2	3812	6	11	NULL	NULL	NULL	Raf-1 peptide	GP		inhibits 		dose-dependently			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_137	15485920	(B) Dose-dependent inhibition of the binding of  Raf-1 to GST-Rb by the Raf-1 peptide in a GST pull-down assay.	bind
81601	1	3812	11	NULL	NULL	0	NULL	Raf-1	GeneOrProtein		binds to 					GST-Rb	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_137	15485920	(B) Dose-dependent inhibition of the binding of  Raf-1 to GST-Rb by the Raf-1 peptide in a GST pull-down assay.	bind
81602	2	3812	11	NULL	NULL	0	NULL	Raf-1 peptide	PartOfProtein		inhibits					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_137	15485920	(B) Dose-dependent inhibition of the binding of  Raf-1 to GST-Rb by the Raf-1 peptide in a GST pull-down assay.	bind
8927	1	3813	5	11	NULL	NULL	NULL	BMP-7	GP	125I-labeled	bind					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_308_4_858_s_197	12927798	(B) Dose-response curve for 125I-labeled BMP-7 binding with heparin.	bind
9203	1	3813	6	11	NULL	NULL	NULL	BMP-7	GP	125I-labeled	bind					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_308_4_858_s_197	12927798	(B) Dose-response curve for 125I-labeled BMP-7 binding with heparin.	bind
81603	1	3813	11	NULL	NULL	0	NULL	BMP-7	GeneOrProtein	125I-labeled	binds to 					heparin	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_308_4_858_s_197	12927798	(B) Dose-response curve for 125I-labeled BMP-7 binding with heparin.	bind
8928	1	3814	5	11	NULL	NULL	NULL	FASII	GP		bind			C-terminal 98-amino-acid residues		DLG	GP		PDZ domains		NULL		NULL	NULL	NULL	NULL	gw60_neuron_19_4_787_s_155	9354326	(B) Dose-response curves of C-terminal 98-amino-acid residues of FASII binding to the PDZ domains in DLG and SAP97.	bind
8929	2	3814	5	11	NULL	NULL	NULL	FASII	GP		bind			C-terminal 98-amino-acid residues		SAP97	GP		PDZ domain		NULL		NULL	NULL	NULL	NULL	gw60_neuron_19_4_787_s_155	9354326	(B) Dose-response curves of C-terminal 98-amino-acid residues of FASII binding to the PDZ domains in DLG and SAP97.	bind
9204	1	3814	6	11	NULL	NULL	NULL	FASII	GP		bind			C-terminal 98-amino-acid residues		DLG	GP		PDZ domain		NULL		NULL	NULL	NULL	NULL	gw60_neuron_19_4_787_s_155	9354326	(B) Dose-response curves of C-terminal 98-amino-acid residues of FASII binding to the PDZ domains in DLG and SAP97.	bind
9205	2	3814	6	11	NULL	NULL	NULL	FASII	GP		bind			C-terminal 98-amino-acid residues		SAP97	GP		PDZ domain		NULL		NULL	NULL	NULL	NULL	gw60_neuron_19_4_787_s_155	9354326	(B) Dose-response curves of C-terminal 98-amino-acid residues of FASII binding to the PDZ domains in DLG and SAP97.	bind
81604	1	3814	11	NULL	NULL	0	NULL	FASII	Protein		binds to 			C-terminal 98-amino-acid		DLG	Protein		PDZ domain		NULL		0	NULL	NULL	NULL	gw60_neuron_19_4_787_s_155	9354326	(B) Dose-response curves of C-terminal 98-amino-acid residues of FASII binding to the PDZ domains in DLG and SAP97.	bind
81605	2	3814	11	NULL	NULL	0	NULL	FASII	Protein		binds to 			C-terminal 98-amino-acid		SAP97	Protein		PDZ domain		NULL		0	NULL	NULL	NULL	gw60_neuron_19_4_787_s_155	9354326	(B) Dose-response curves of C-terminal 98-amino-acid residues of FASII binding to the PDZ domains in DLG and SAP97.	bind
8930	1	3816	5	11	NULL	NULL	NULL	Hsp70	GP		bind					PBMC	Cell	human			NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_3_353_s_37	12354387	(B) Dot plot profile showing the binding of Hsp70 to human PBMC.	bind
9206	1	3816	6	11	NULL	NULL	NULL	Hsp70	GP		bind					PBMC	Cell	human			NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_3_353_s_37	12354387	(B) Dot plot profile showing the binding of Hsp70 to human PBMC.	bind
81606	1	3816	11	NULL	NULL	0	NULL	Hsp70	GeneOrProtein		binds to 					PBMC	Cell	human			NULL		0	NULL	NULL	NULL	gw60_immunity_17_3_353_s_37	12354387	(B) Dot plot profile showing the binding of Hsp70 to human PBMC.	bind
8931	1	3817	5	11	NULL	NULL	NULL	TBPCORE	GP	human	bind					 DNA	NucleicAcid			TATA box	NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_1_151_s_77	12535529	(B) Downstream or front view of the human TBPCORE (white) bound to the TATA box-containing DNA (green)  (Nikolov et al., 1996  ).	bind
9207	1	3817	6	11	NULL	NULL	NULL	TBPCORE	GP	human	bind					DNA	NucleicAcid			TATA box	NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_1_151_s_77	12535529	(B) Downstream or front view of the human TBPCORE (white) bound to the TATA box-containing DNA (green)  (Nikolov et al., 1996  ).	bind
81607	1	3817	11	NULL	NULL	0	NULL	TBPCORE	GeneOrProtein	Human	binds to 					DNA	NucleicAcidSubstance	TATA box			NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_151_s_77	12535529	(B) Downstream or front view of the human TBPCORE (white) bound to the TATA box-containing DNA (green)  (Nikolov et al., 1996  ).	bind
8932	1	3819	5	11	NULL	NULL	NULL	GFP - X-PAK5	GP		bind					MTs	CellComponent				NULL	live A6 cells	NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_1029_s_210	11733543	(B) Dynamics of GFP - X-PAK5 - bound MTs in live A6 cells.	bind
9208	1	3819	6	11	NULL	NULL	NULL	GFP - X-PAK5	GP		bind					MTs	CellComponent				NULL	live A6 cells	NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_1029_s_210	11733543	(B) Dynamics of GFP - X-PAK5 - bound MTs in live A6 cells.	bind
81608	1	3819	11	NULL	NULL	0	NULL	GFP - X-PAK5	GeneOrProtein		binds to 					MT	CellComponent	live A6 cell			NULL		0	NULL	NULL	NULL	gw60_cellbiol_155_6_1029_s_210	11733543	(B) Dynamics of GFP - X-PAK5 - bound MTs in live A6 cells.	bind
8933	1	3820	5	11	NULL	NULL	NULL	E2F-4	GP		bind					p130	GP				NULL	insect cell lysate expressing p130,E2F-4,DP-1	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6233_s_31	10938100	(B) E2F-4 is bound to p130 in insect cell lysate expressing p130, E2F-4, and DP-1.	bind
9241	1	3820	6	11	NULL	NULL	NULL	E2F-4	GP		bind					p130	GP				NULL	insect cell lysate expressing p130,E2F-4,DP-1	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6233_s_31	10938100	(B) E2F-4 is bound to p130 in insect cell lysate expressing p130, E2F-4, and DP-1.	bind
81609	1	3820	11	NULL	NULL	0	NULL	E2F-4	GeneOrProtein		binds to 					p130	GeneOrProtein	insect cell lysate			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_17_6233_s_31	10938100	(B) E2F-4 is bound to p130 in insect cell lysate expressing p130, E2F-4, and DP-1.	bind
81610	2	3820	11	NULL	NULL	0	NULL	insect cell	cell		express					p130	Gene				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_17_6233_s_31	10938100	(B) E2F-4 is bound to p130 in insect cell lysate expressing p130, E2F-4, and DP-1.	bind
81611	3	3820	11	NULL	NULL	0	NULL	insect cell	cell		express					E2F-4	Gene				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_17_6233_s_31	10938100	(B) E2F-4 is bound to p130 in insect cell lysate expressing p130, E2F-4, and DP-1.	bind
81612	4	3820	11	NULL	NULL	0	NULL	insect cell	cell		express					DP-1	Gene				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_17_6233_s_31	10938100	(B) E2F-4 is bound to p130 in insect cell lysate expressing p130, E2F-4, and DP-1.	bind
8936	1	3821	5	11	NULL	NULL	NULL	E64	Chemical		stabilize					FH	GP	binding activity of			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_11_6206_s_299	12379699	(B) E64 stabilizes FH binding activity.	bind
9245	1	3821	6	11	NULL	NULL	NULL	E64	Chemical		stabilizes					FH	GP	binding activity of 			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_11_6206_s_299	12379699	(B) E64 stabilizes FH binding activity.	bind
81613	1	3821	11	NULL	NULL	0	NULL	E64	Chemical		stabilizes					FH	GeneOrProtein	binding activity			NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_11_6206_s_299	12379699	(B) E64 stabilizes FH binding activity.	bind
8937	1	3822	5	11	NULL	NULL	NULL	cIR-MAP2c (-Au11)	GP	unlabeled	bind					2.6 tubulin monomers	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_7_1187_s_103	12082079	(B) Each unlabeled cIR-MAP2c (-Au11) bound 2.6 tubulin monomers and each gold-labeled cIR-MAP2c (+Au11) bound 2.5 tubulin monomers.	bind
8938	2	3822	5	11	NULL	NULL	NULL	IR-MAP2c (+Au11)	GP	gold-labeled	bind					2.5 tubulin monomers	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_7_1187_s_103	12082079	(B) Each unlabeled cIR-MAP2c (-Au11) bound 2.6 tubulin monomers and each gold-labeled cIR-MAP2c (+Au11) bound 2.5 tubulin monomers.	bind
9246	1	3822	6	11	NULL	NULL	NULL	cIR-MAP2c	GP	unlabeled	bind					2.6 tubulin monomer	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_7_1187_s_103	12082079	(B) Each unlabeled cIR-MAP2c (-Au11) bound 2.6 tubulin monomers and each gold-labeled cIR-MAP2c (+Au11) bound 2.5 tubulin monomers.	bind
9247	2	3822	6	11	NULL	NULL	NULL	cIR-MAP2c	GP	gold labeled	bind					2.5 tubulin monomer	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_7_1187_s_103	12082079	(B) Each unlabeled cIR-MAP2c (-Au11) bound 2.6 tubulin monomers and each gold-labeled cIR-MAP2c (+Au11) bound 2.5 tubulin monomers.	bind
81614	1	3822	11	NULL	NULL	NULL	NULL	cIR-MAP2c	GeneOrProtein	unlabeled	binds to 					2.6 tubulin monomer	Protein				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_7_1187_s_103	12082079	(B) Each unlabeled cIR-MAP2c (-Au11) bound 2.6 tubulin monomers and each gold-labeled cIR-MAP2c (+Au11) bound 2.5 tubulin monomers.	bind
81615	2	3822	11	NULL	NULL	0	NULL	cIR-MAP2c	GeneOrProtein	gold-labeled	binds to 					2.5 tubulin monomer	Protein				NULL		0	NULL	NULL	NULL	gw60_cellbiol_157_7_1187_s_103	12082079	(B) Each unlabeled cIR-MAP2c (-Au11) bound 2.6 tubulin monomers and each gold-labeled cIR-MAP2c (+Au11) bound 2.5 tubulin monomers.	bind
8939	1	3823	5	11	NULL	NULL	NULL	EBAG9	GP		bind			predicted TM region		Snapin	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_3_1245_s_200	15635093	(B) EBAG9 binds to Snapin via  its predicted TM region.	bind
9249	1	3823	6	11	NULL	NULL	NULL	EBAG9	GP		bind			predicted TM region		Snapin	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_3_1245_s_200	15635093	(B) EBAG9 binds to Snapin via  its predicted TM region.	bind
81616	1	3823	11	NULL	NULL	0	NULL	EBAG9	Gene		binds to 				TM region	Snapin	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_3_1245_s_200	15635093	(B) EBAG9 binds to Snapin via  its predicted TM region.	bind
8941	1	3824	5	11	NULL	NULL	NULL	Ecm22p	GP		bind		directly			ERG2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6395_s_273	11533229	(B) Ecm22p also bound directly to the  ERG2 promoter in a SRE-dependent manner.	bind
8942	2	3824	5	11	NULL	NULL	NULL	statement 1	Process		is dependent on									SRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6395_s_273	11533229	(B) Ecm22p also bound directly to the  ERG2 promoter in a SRE-dependent manner.	bind
9250	1	3824	6	11	NULL	NULL	NULL	Ecm22p	GP		bind		directly			ERG2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6395_s_273	11533229	(B) Ecm22p also bound directly to the  ERG2 promoter in a SRE-dependent manner.	bind
9251	2	3824	6	11	NULL	NULL	NULL	statement 1	Process		is dependent on									SRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6395_s_273	11533229	(B) Ecm22p also bound directly to the  ERG2 promoter in a SRE-dependent manner.	bind
81617	1	3824	11	NULL	NULL	0	NULL	Ecm22p	Protein		binds to 		directly			ERG2	Gene			promoter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_19_6395_s_273	11533229	(B) Ecm22p also bound directly to the  ERG2 promoter in a SRE-dependent manner.	bind
81618	2	3824	11	NULL	NULL	0	NULL	statement 1	Process		depends on					SRE	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_19_6395_s_273	11533229	(B) Ecm22p also bound directly to the  ERG2 promoter in a SRE-dependent manner.	bind
8943	1	3825	5	11	NULL	NULL	NULL	Ras	GP	inhibition of	induce					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_24_9271_s_220	11094078	(B) Ectopic expression of  bcl-2 blocks apoptosis induced by inhibition of Ras and PI 3-kinase.	bind
8944	2	3825	5	11	NULL	NULL	NULL	PI 3-kinase	GP	inhibition of	induce					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_24_9271_s_220	11094078	(B) Ectopic expression of  bcl-2 blocks apoptosis induced by inhibition of Ras and PI 3-kinase.	bind
8945	3	3825	5	11	NULL	NULL	NULL	 bcl-2	GP	ectopic expression of	blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_24_9271_s_220	11094078	(B) Ectopic expression of  bcl-2 blocks apoptosis induced by inhibition of Ras and PI 3-kinase.	bind
8946	4	3825	5	11	NULL	NULL	NULL	bcl-2	GP	ectopic expression of	blocks					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_24_9271_s_220	11094078	(B) Ectopic expression of  bcl-2 blocks apoptosis induced by inhibition of Ras and PI 3-kinase.	bind
9252	1	3825	6	11	NULL	NULL	NULL	Ras	GP	inhibition of	induces					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_24_9271_s_220	11094078	(B) Ectopic expression of  bcl-2 blocks apoptosis induced by inhibition of Ras and PI 3-kinase.	bind
9253	2	3825	6	11	NULL	NULL	NULL	PI 3-kinase	GP	inhibition of	induces					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_24_9271_s_220	11094078	(B) Ectopic expression of  bcl-2 blocks apoptosis induced by inhibition of Ras and PI 3-kinase.	bind
9254	3	3825	6	11	NULL	NULL	NULL	Bcl-2	GP	ectopic expression of	blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_24_9271_s_220	11094078	(B) Ectopic expression of  bcl-2 blocks apoptosis induced by inhibition of Ras and PI 3-kinase.	bind
9255	4	3825	6	11	NULL	NULL	NULL	Bcl-2	GP	ectopic expression of	blocks					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_24_9271_s_220	11094078	(B) Ectopic expression of  bcl-2 blocks apoptosis induced by inhibition of Ras and PI 3-kinase.	bind
81619	1	3825	11	NULL	NULL	0	NULL	bcl-2	GeneOrProtein	Ectopic expression	blocks					apoptosis	BiologicalProcess				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_24_9271_s_220	11094078	(B) Ectopic expression of  bcl-2 blocks apoptosis induced by inhibition of Ras and PI 3-kinase.	bind
81620	2	3825	11	NULL	NULL	0	NULL	Ras	GeneOrProtein	inhibition	induces					apoptosis	BiologicalProcess				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_24_9271_s_220	11094078	(B) Ectopic expression of  bcl-2 blocks apoptosis induced by inhibition of Ras and PI 3-kinase.	bind
81621	3	3825	11	NULL	NULL	0	NULL	PI 3-kinase	GeneOrProtein	inhibition	induces					apoptosis	BiologicalProcess				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_24_9271_s_220	11094078	(B) Ectopic expression of  bcl-2 blocks apoptosis induced by inhibition of Ras and PI 3-kinase.	bind
8947	1	3826	5	11	NULL	NULL	NULL	NF-kappaB	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_1_206_s_140	9864217	(B) Effect of antibodies against TNF-alpha or IL-1R on the induction of DNA binding of NF-kappaB by LPS with or without priming by IFN-gamma.	bind
8948	2	3826	5	11	NULL	NULL	NULL	LPS	Chemical		induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_1_206_s_140	9864217	(B) Effect of antibodies against TNF-alpha or IL-1R on the induction of DNA binding of NF-kappaB by LPS with or without priming by IFN-gamma.	bind
9256	1	3826	6	11	NULL	NULL	NULL	NF-kappaB	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_1_206_s_140	9864217	(B) Effect of antibodies against TNF-alpha or IL-1R on the induction of DNA binding of NF-kappaB by LPS with or without priming by IFN-gamma.	bind
9257	2	3826	6	11	NULL	NULL	NULL	LPS	Chemical		induces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_1_206_s_140	9864217	(B) Effect of antibodies against TNF-alpha or IL-1R on the induction of DNA binding of NF-kappaB by LPS with or without priming by IFN-gamma.	bind
81622	1	3826	11	NULL	NULL	0	NULL	NF-kappaB	Protein		binds to 					DNA	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw60_infectimmun_67_1_206_s_140	9864217	(B) Effect of antibodies against TNF-alpha or IL-1R on the induction of DNA binding of NF-kappaB by LPS with or without priming by IFN-gamma.	bind
81623	2	3826	11	NULL	NULL	0	NULL	LPS	NonProteinOrNucleicAcidChemical		induces					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_infectimmun_67_1_206_s_140	9864217	(B) Effect of antibodies against TNF-alpha or IL-1R on the induction of DNA binding of NF-kappaB by LPS with or without priming by IFN-gamma.	bind
8949	1	3827	5	11	NULL	NULL	NULL	syntaxin	GP		bind					synaptotagmin	GP		C2A domain		NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_86_1_39_s_133	9692742	(B) Effect of antibodies on Ca2+-dependent syntaxin binding to synaptotagmin C2A domain.	bind
8950	2	3827	5	11	NULL	NULL	NULL	statement 1	Process		is dependent on					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_86_1_39_s_133	9692742	(B) Effect of antibodies on Ca2+-dependent syntaxin binding to synaptotagmin C2A domain.	bind
9258	1	3827	6	11	NULL	NULL	NULL	syntaxin	GP		bind					synaptotagmin	GP		C2A domain		NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_86_1_39_s_133	9692742	(B) Effect of antibodies on Ca2+-dependent syntaxin binding to synaptotagmin C2A domain.	bind
9259	2	3827	6	11	NULL	NULL	NULL	statement 1	Process		is dependent on					Ca+2	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_86_1_39_s_133	9692742	(B) Effect of antibodies on Ca2+-dependent syntaxin binding to synaptotagmin C2A domain.	bind
81624	1	3827	11	NULL	NULL	NULL	NULL	syntaxin	GeneOrProtein		binds to 					synaptotagmin	Protein		C2A domain		NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_86_1_39_s_133	9692742	(B) Effect of antibodies on Ca2+-dependent syntaxin binding to synaptotagmin C2A domain.	bind
81625	2	3827	11	NULL	NULL	0	NULL	statement 1	Process		depends on					Ca2+	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	gw60_neuroscience_86_1_39_s_133	9692742	(B) Effect of antibodies on Ca2+-dependent syntaxin binding to synaptotagmin C2A domain.	bind
8951	1	3828	5	11	NULL	NULL	NULL	dynein	GP		bind					liposomes	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_1_173_s_74	11172722	(B) Effect of antibodies on the binding of dynein and dynactin to liposomes.	bind
8952	2	3828	5	11	NULL	NULL	NULL	dynactin	GP		bind					liposomes	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_1_173_s_74	11172722	(B) Effect of antibodies on the binding of dynein and dynactin to liposomes.	bind
9260	1	3828	6	11	NULL	NULL	NULL	dynein	GP		bind					liposomes	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_1_173_s_74	11172722	(B) Effect of antibodies on the binding of dynein and dynactin to liposomes.	bind
9261	2	3828	6	11	NULL	NULL	NULL	dynactin	GP		bind					liposomes	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_1_173_s_74	11172722	(B) Effect of antibodies on the binding of dynein and dynactin to liposomes.	bind
81626	1	3828	11	NULL	NULL	0	NULL	 dynein	Protein		binds to 					liposomes	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	gw60_molcell_7_1_173_s_74	11172722	(B) Effect of antibodies on the binding of dynein and dynactin to liposomes.	bind
81627	2	3828	11	NULL	NULL	0	NULL	dynactin	Protein		binds to 					liposomes	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	gw60_molcell_7_1_173_s_74	11172722	(B) Effect of antibodies on the binding of dynein and dynactin to liposomes.	bind
8953	1	3829	5	11	NULL	NULL	NULL	tubulin	GP		bind					colchicine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1432_2_350_s_114	10407156	(B) Effect of bisANS and GTP on the colchicine binding activity of tubulin.	bind
9262	1	3829	6	11	NULL	NULL	NULL	tubulin	GP		bind					colchicine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1432_2_350_s_114	10407156	(B) Effect of bisANS and GTP on the colchicine binding activity of tubulin.	bind
81628	1	3829	11	NULL	NULL	0	NULL	colchicine	NonProteinOrNucleicAcidChemical		binds to 					tubulin	Protein				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1432_2_350_s_114	10407156	(B) Effect of bisANS and GTP on the colchicine binding activity of tubulin.	bind
8954	1	3830	5	11	NULL	NULL	NULL	AFP	GP		bind					MDM	Cell				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_3_507_s_103	12176010	(B) Effect of bovine fetuin (500 nM) (AFP + fetuin) or AGP (AFP + AGP) on [125]AFP binding to MDM (AFP).	bind
9263	1	3830	6	11	NULL	NULL	NULL	AFP	GP		bind					MDM	Cell				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_3_507_s_103	12176010	(B) Effect of bovine fetuin (500 nM) (AFP + fetuin) or AGP (AFP + AGP) on [125]AFP binding to MDM (AFP).	bind
81629	1	3830	11	NULL	NULL	0	NULL	AFP	Protein		binds to 					MDM	Cell				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_3_507_s_103	12176010	(B) Effect of bovine fetuin (500 nM) (AFP + fetuin) or AGP (AFP + AGP) on [125]AFP binding to MDM (AFP).	bind
8955	1	3831	5	11	NULL	NULL	NULL	C5	GP		bind					GST-p16	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_3_421_s_182	9660926	(B) Effect of R24C mutation on the binding of C5 to GST-p16.	bind
9264	1	3831	6	11	NULL	NULL	NULL	C5	GP		bind					GST-p16	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_3_421_s_182	9660926	(B) Effect of R24C mutation on the binding of C5 to GST-p16.	bind
81630	1	3831	11	NULL	NULL	0	NULL	C5	Protein		binds to 					 GST-p16	Protein				NULL		0	NULL	NULL	NULL	gw60_molcell_1_3_421_s_182	9660926	(B) Effect of R24C mutation on the binding of C5 to GST-p16.	bind
8956	1	3832	5	11	NULL	NULL	NULL	p97	GP		bind					p62	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_8_12_2379_s_193	9398662	(B) Effect of Ran on the binding of p97 to p62.	bind
9265	1	3832	6	11	NULL	NULL	NULL	p97	GP		bind					p62	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_8_12_2379_s_193	9398662	(B) Effect of Ran on the binding of p97 to p62.	bind
81631	1	3832	11	NULL	NULL	0	NULL	p97	GeneOrProtein		binds to 					p62	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_8_12_2379_s_193	9398662	(B) Effect of Ran on the binding of p97 to p62.	bind
8957	1	3833	5	11	NULL	NULL	NULL	Bas2p	GP		bind					Bas1p	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_23_7901_s_330	11689683	(B) Effect of SAICAR and AICAR on in vitro binding of Bas2p to Bas1p on the  ADE5,7 promoter.	bind
13173	2	3833	5	11	NULL	NULL	NULL	statement 1	GP		bind					ADE5,7	GP			promoter	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_23_7901_s_330	11689683	(B) Effect of SAICAR and AICAR on in vitro binding of Bas2p to Bas1p on the  ADE5,7 promoter.	bind
9266	1	3833	6	11	NULL	NULL	NULL	Bas2p	GP		bind					Bas1p	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_23_7901_s_330	11689683	(B) Effect of SAICAR and AICAR on in vitro binding of Bas2p to Bas1p on the  ADE5,7 promoter.	bind
11761	2	3833	6	11	NULL	NULL	NULL	statement 1	GP		binds					ADE5,7	GP			promoter	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_23_7901_s_330	11689683	(B) Effect of SAICAR and AICAR on in vitro binding of Bas2p to Bas1p on the  ADE5,7 promoter.	bind
81632	1	3833	11	NULL	NULL	0	NULL	Bas2p	GeneOrProtein		binds to 					Bas1p	Gene			ADE5,7 promoter	NULL	in vitro	0	NULL	NULL	NULL	gw60_molcellbiol_21_23_7901_s_330	11689683	(B) Effect of SAICAR and AICAR on in vitro binding of Bas2p to Bas1p on the  ADE5,7 promoter.	bind
8958	1	3834	5	11	NULL	NULL	NULL	TN-R 160	GP		bind					FN fragments	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainres_863_1_42_s_111	10773191	(B) Effect of soluble GAGs on the binding of TN-R 160 to FN fragments and heparin-binding peptides.	bind
8959	2	3834	5	11	NULL	NULL	NULL	TN-R 160	GP		bind					heparin-binding peptides	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainres_863_1_42_s_111	10773191	(B) Effect of soluble GAGs on the binding of TN-R 160 to FN fragments and heparin-binding peptides.	bind
9267	1	3834	6	11	NULL	NULL	NULL	TN-R 160	GP		bind					FN fragments	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainres_863_1_42_s_111	10773191	(B) Effect of soluble GAGs on the binding of TN-R 160 to FN fragments and heparin-binding peptides.	bind
9268	2	3834	6	11	NULL	NULL	NULL	heparin	Chemical		bind					peptides	amino acid				NULL		NULL	NULL	NULL	NULL	gw60_brainres_863_1_42_s_111	10773191	(B) Effect of soluble GAGs on the binding of TN-R 160 to FN fragments and heparin-binding peptides.	bind
9269	3	3834	6	11	NULL	NULL	NULL	TN-R 160	GP		bind					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainres_863_1_42_s_111	10773191	(B) Effect of soluble GAGs on the binding of TN-R 160 to FN fragments and heparin-binding peptides.	bind
81633	1	3834	11	NULL	NULL	0	NULL	 TN-R	GeneOrProtein		binds to 					FN fragment	PartOfProtein				NULL		0	NULL	NULL	NULL	gw60_brainres_863_1_42_s_111	10773191	(B) Effect of soluble GAGs on the binding of TN-R 160 to FN fragments and heparin-binding peptides.	bind
81634	2	3834	11	NULL	NULL	0	NULL	TN-R 	GeneOrProtein		binds to 					heparin-binding peptide	PartOfProtein				NULL		0	NULL	NULL	NULL	gw60_brainres_863_1_42_s_111	10773191	(B) Effect of soluble GAGs on the binding of TN-R 160 to FN fragments and heparin-binding peptides.	bind
8960	1	3835	5	11	NULL	NULL	NULL	TN-R 160	GP		bind					TN-C	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainres_863_1_42_s_143	10773191	(B) Effect of soluble GAGs on the binding of TN-R 160 to TN-C.	bind
9270	1	3835	6	11	NULL	NULL	NULL	TN-R 160	GP		bind					TN-C	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainres_863_1_42_s_143	10773191	(B) Effect of soluble GAGs on the binding of TN-R 160 to TN-C.	bind
81635	1	3835	11	NULL	NULL	0	NULL	TN-R 160	GeneOrProtein		binds to 					TN-C	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_brainres_863_1_42_s_143	10773191	(B) Effect of soluble GAGs on the binding of TN-R 160 to TN-C.	bind
8961	1	3836	5	11	NULL	NULL	NULL	Css IV	GP		bind					rIIA 	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_4_919_s_145	9808476	(B) Effect of the different mutations on Css IV binding affinity to rIIA sodium channels.	bind
53645	2	3836	5	11	NULL	NULL	NULL	rIIA	GP		is a type of					sodium channel	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_4_919_s_145	9808476	(B) Effect of the different mutations on Css IV binding affinity to rIIA sodium channels.	bind
9271	1	3836	6	11	NULL	NULL	NULL	Css IV	GP		bind					rIIA	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_4_919_s_145	9808476	(B) Effect of the different mutations on Css IV binding affinity to rIIA sodium channels.	bind
41010	2	3836	6	11	NULL	NULL	NULL	rIIA	GP		is a type of					sodium channel	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_4_919_s_145	9808476	(B) Effect of the different mutations on Css IV binding affinity to rIIA sodium channels.	bind
81636	1	3836	11	NULL	NULL	0	NULL	Css IV	GeneOrProtein		binds to 					rIIA 	GeneOrProtein	sodium channels			NULL		0	NULL	NULL	NULL	gw60_neuron_21_4_919_s_145	9808476	(B) Effect of the different mutations on Css IV binding affinity to rIIA sodium channels.	bind
8962	1	3837	5	11	NULL	NULL	NULL	GTP	Chemical		bind					His6-BCTD	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_6_1347_s_153	9515899	(B) Effect on the GTP binding of His6-BCTD.	bind
9272	1	3837	6	11	NULL	NULL	NULL	His6-BCTD	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_6_1347_s_153	9515899	(B) Effect on the GTP binding of His6-BCTD.	bind
81637	1	3837	11	NULL	NULL	0	NULL	His6-BCTD	Protein		binds to 					GTP	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_6_1347_s_153	9515899	(B) Effect on the GTP binding of His6-BCTD.	bind
8963	1	3838	5	11	NULL	NULL	NULL	NSAP1	GP	purified	bind					probe IV	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_18_7878_s_117	15340051	(B) Effects of competitor RNAs on binding of purified NSAP1 to probe  IV.	bind
9273	1	3838	6	11	NULL	NULL	NULL	NSAP1	GP	purified	bind					probe IV	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_18_7878_s_117	15340051	(B) Effects of competitor RNAs on binding of purified NSAP1 to probe  IV.	bind
81638	1	3838	11	NULL	NULL	0	NULL	NSAP1	GeneOrProtein		binds to 					probe IV	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_18_7878_s_117	15340051	(B) Effects of competitor RNAs on binding of purified NSAP1 to probe  IV.	bind
8964	1	3839	5	11	NULL	NULL	NULL	MAb	GP		bind					O-PG	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_clindiagnlabimmun_8_3_647_s_75	11329475	(B) Effects of fungal glucan on MAb binding to O-PG-coated wells.	bind
9274	1	3839	6	11	NULL	NULL	NULL	MAb	GP		bind 					O-PG	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_clindiagnlabimmun_8_3_647_s_75	11329475	(B) Effects of fungal glucan on MAb binding to O-PG-coated wells.	bind
81639	1	3839	11	NULL	NULL	0	NULL	MAb	Protein		binds to 					O-PG	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	gw60_clindiagnlabimmun_8_3_647_s_75	11329475	(B) Effects of fungal glucan on MAb binding to O-PG-coated wells.	bind
8965	1	3840	5	11	NULL	NULL	NULL	Gab1	GP		undergoes					phosphorylation	Process		tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_1_103_s_62	12370245	(b) EGF selectively enhances Gab1 tyrosine phosphorylation and binding to SHP-2.	bind
8966	2	3840	5	11	NULL	NULL	NULL	Gab1	GP		bind					SHP-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_1_103_s_62	12370245	(b) EGF selectively enhances Gab1 tyrosine phosphorylation and binding to SHP-2.	bind
8967	3	3840	5	11	NULL	NULL	NULL	EGF	GP		enhances		selectively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_1_103_s_62	12370245	(b) EGF selectively enhances Gab1 tyrosine phosphorylation and binding to SHP-2.	bind
8968	4	3840	5	11	NULL	NULL	NULL	EGF	GP		enhances		selectively			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_1_103_s_62	12370245	(b) EGF selectively enhances Gab1 tyrosine phosphorylation and binding to SHP-2.	bind
9275	1	3840	6	11	NULL	NULL	NULL	Gab1	GP		bind					SHP-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_1_103_s_62	12370245	(b) EGF selectively enhances Gab1 tyrosine phosphorylation and binding to SHP-2.	bind
9276	2	3840	6	11	NULL	NULL	NULL	EGF	GP		enhances		selectively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_1_103_s_62	12370245	(b) EGF selectively enhances Gab1 tyrosine phosphorylation and binding to SHP-2.	bind
9277	4	3840	6	11	NULL	NULL	NULL	EGF	GP		enhances		selectively			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_1_103_s_62	12370245	(b) EGF selectively enhances Gab1 tyrosine phosphorylation and binding to SHP-2.	bind
53647	3	3840	6	11	NULL	NULL	NULL	Gab1	GP		undergoes					phosphorylation	Process		tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_1_103_s_62	12370245	(b) EGF selectively enhances Gab1 tyrosine phosphorylation and binding to SHP-2.	bind
81640	1	3840	11	NULL	NULL	0	NULL	Gab1	Protein	tyrosine phosphorylate	binds to 					SHP-2	GeneOrProtein				NULL		0	NULL	NULL	NULL	gw60_cellbiol_159_1_103_s_62	12370245	(b) EGF selectively enhances Gab1 tyrosine phosphorylation and binding to SHP-2.	bind
81641	2	3840	11	NULL	NULL	0	NULL	EGF	Protein		enhances		selectively			statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_159_1_103_s_62	12370245	(b) EGF selectively enhances Gab1 tyrosine phosphorylation and binding to SHP-2.	bind
9386	1	3841	5	11	NULL	NULL	NULL	GDP	Chemical		bind					eIF2	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1492_1_56_s_172	10858531	(B) eIF2B activity was analyzed in lysates from infected Sf9 cells as described in A. Aliquots (40  l) of lysates containing wild-type AcNPV baculovirus (AcNPV), five subunit eIF2B with wild-type (lane 1, GST 1-716) and truncated (lane 2, GST 1-164; lane 3, GST 159-716) GST-eIF2B  fusion proteins were assayed for guanine nucleotide exchange activity, measured as the exchange of [3]GDP bound to eIF2 for nonradiolabeled GDP over time.	bind
9357	1	3841	6	11	NULL	NULL	NULL	GDP	Chemical		bind					eIF2	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1492_1_56_s_172	10858531	(B) eIF2B activity was analyzed in lysates from infected Sf9 cells as described in A. Aliquots (40  l) of lysates containing wild-type AcNPV baculovirus (AcNPV), five subunit eIF2B with wild-type (lane 1, GST 1-716) and truncated (lane 2, GST 1-164; lane 3, GST 159-716) GST-eIF2B  fusion proteins were assayed for guanine nucleotide exchange activity, measured as the exchange of [3]GDP bound to eIF2 for nonradiolabeled GDP over time.	bind
81642	1	3841	11	NULL	NULL	0	NULL	GDP	NonProteinOrNucleicAcidChemical		binds to 					eIF2	Protein				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1492_1_56_s_172	10858531	(B) eIF2B activity was analyzed in lysates from infected Sf9 cells as described in A. Aliquots (40  l) of lysates containing wild-type AcNPV baculovirus (AcNPV), five subunit eIF2B with wild-type (lane 1, GST 1-716) and truncated (lane 2, GST 1-164; lane 3, GST 159-716) GST-eIF2B  fusion proteins were assayed for guanine nucleotide exchange activity, measured as the exchange of [3]GDP bound to eIF2 for nonradiolabeled GDP over time.	bind
8969	1	3842	5	11	NULL	NULL	NULL	TFIIB	GP		bind							unbent		TBP-TATA box complex	NULL		NULL	NULL	NULL	NULL	gw60_cell_108_5_615_s_202	11893333	(B) Electrophoretic mobility retardation analysis of TFIIB binding to the unbent TBP-TATA box complex.	bind
9364	1	3842	6	11	NULL	NULL	NULL	TFIIB	GP		bind							unbent		TBP-TATA box complex	NULL		NULL	NULL	NULL	NULL	gw60_cell_108_5_615_s_202	11893333	(B) Electrophoretic mobility retardation analysis of TFIIB binding to the unbent TBP-TATA box complex.	bind
81643	1	3842	11	NULL	NULL	0	NULL	TFIIB	GeneOrProtein		binds to 					TBP-TATA box	GeneOrProtein	unbent			NULL		0	NULL	NULL	NULL	gw60_cell_108_5_615_s_202	11893333	(B) Electrophoretic mobility retardation analysis of TFIIB binding to the unbent TBP-TATA box complex.	bind
8970	1	3843	5	11	NULL	NULL	NULL	Atf1pHa	GP		bind					ntp1+	GP			CRE element at promoter	NULL		NULL	NULL	NULL	NULL	gw70_yeast_21_7_593_s_145	15164362	(B) EMSA analysis of Atf1pHa binding to CRE element at  ntp1+ promoter.	bind
9365	1	3843	6	11	NULL	NULL	NULL	Atf1pHa	GP		bind					ntp1+	GP			CRE element of promoter	NULL		NULL	NULL	NULL	NULL	gw70_yeast_21_7_593_s_145	15164362	(B) EMSA analysis of Atf1pHa binding to CRE element at  ntp1+ promoter.	bind
81644	1	3843	11	NULL	NULL	0	NULL	Atf1pHa	GeneOrProtein		binds to 					CRE	Gene			ntp1+ promoter	NULL		0	NULL	NULL	NULL	gw70_yeast_21_7_593_s_145	15164362	(B) EMSA analysis of Atf1pHa binding to CRE element at  ntp1+ promoter.	bind
8971	1	3844	5	11	NULL	NULL	NULL	MEF2C	GP		bind					CRT	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_170_1_37_s_163	15998798	(B) EMSA analysis of MEF2C binding to the CRT promoter.	bind
9366	1	3844	6	11	NULL	NULL	NULL	MEF2C	GP		bind					CRT	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_170_1_37_s_163	15998798	(B) EMSA analysis of MEF2C binding to the CRT promoter.	bind
81645	1	3844	11	NULL	NULL	0	NULL	MEF2C	GeneOrProtein		binds to 					CRT	Gene			promoter	NULL		0	NULL	NULL	NULL	gw70_cellbiol_170_1_37_s_163	15998798	(B) EMSA analysis of MEF2C binding to the CRT promoter.	bind
9439	1	3845	5	11	NULL	NULL	NULL	p53	GP		bind					DNA	NucleicAcid				NULL	whole cell extracts from Rb/ ARF E13.5 brains	NULL	NULL	NULL	NULL	gw60_currbiol_12_2_159_s_74	11818069	(B) EMSA demonstrates that  p53 DNA binding activity in whole cell extracts from  Rb/ ARF E13.5 brains using a radiolabeled  p53 consensus binding site oligonucleotide is upregulated (lanes 11 and 12) compared to wild-type controls (lanes 3 and 4) and comparable to levels observed in  Rb mutant samples (lanes 7 and 8).	bind
9367	1	3845	6	11	NULL	NULL	NULL	p53	GP		bind					DNA	NucleicAcid				NULL	whole cell extracts from Rb/ ARF E13.5 brains	NULL	NULL	NULL	NULL	gw60_currbiol_12_2_159_s_74	11818069	(B) EMSA demonstrates that  p53 DNA binding activity in whole cell extracts from  Rb/ ARF E13.5 brains using a radiolabeled  p53 consensus binding site oligonucleotide is upregulated (lanes 11 and 12) compared to wild-type controls (lanes 3 and 4) and comparable to levels observed in  Rb mutant samples (lanes 7 and 8).	bind
8972	1	3846	5	11	NULL	NULL	NULL	DAF-16	GP		bind		specifically			daf-15 	GP			IRS	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_development_131_16_3897_s_201	15253933	(B) EMSA indicates DAF-16 binds specifically to the  daf-15 IRS in vitro (see text).	bind
9368	1	3846	6	11	NULL	NULL	NULL	DAF-16	GP		bind		specifically			daf-15	GP			IRS	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_development_131_16_3897_s_201	15253933	(B) EMSA indicates DAF-16 binds specifically to the  daf-15 IRS in vitro (see text).	bind
81646	1	3846	11	NULL	NULL	0	NULL	DAF-16	GeneOrProtein		binds to 					daf-15 IRS	GeneOrProtein				NULL	in vitro	0	NULL	NULL	NULL	gw70_development_131_16_3897_s_201	15253933	(B) EMSA indicates DAF-16 binds specifically to the  daf-15 IRS in vitro (see text).	bind
8973	1	3849	5	11	NULL	NULL	NULL	GRBP	GP	purified;; cytosolic	bind					DNA	NucleicAcid			GRE	NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1624_1_29_s_151	14642810	(B) EMSA of purified cytosolic GRBP and expressed  Translin binding to GRE (MLTF-like site) DNA.	bind
8974	2	3849	5	11	NULL	NULL	NULL	Translin	GP	expressed	bind					DNA	NucleicAcid			GRE	NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1624_1_29_s_151	14642810	(B) EMSA of purified cytosolic GRBP and expressed  Translin binding to GRE (MLTF-like site) DNA.	bind
53648	3	3849	5	11	NULL	NULL	NULL	GRE	GP		is					MLTF-like site	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1624_1_29_s_151	14642810	(B) EMSA of purified cytosolic GRBP and expressed  Translin binding to GRE (MLTF-like site) DNA.	bind
9369	1	3849	6	11	NULL	NULL	NULL	GRBP	GP	purified;; cytosolic	bind					DNA	NucleicAcid			GRE	NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1624_1_29_s_151	14642810	(B) EMSA of purified cytosolic GRBP and expressed  Translin binding to GRE (MLTF-like site) DNA.	bind
9370	2	3849	6	11	NULL	NULL	NULL	translin	GP		bind					DNA	NucleicAcid			GRE	NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1624_1_29_s_151	14642810	(B) EMSA of purified cytosolic GRBP and expressed  Translin binding to GRE (MLTF-like site) DNA.	bind
9371	3	3849	6	11	NULL	NULL	NULL	GRE	GP		is					MLTF-like site	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1624_1_29_s_151	14642810	(B) EMSA of purified cytosolic GRBP and expressed  Translin binding to GRE (MLTF-like site) DNA.	bind
8975	1	3850	5	11	NULL	NULL	NULL	Stat5	GP		bind					BCL-X gene	GP	human		BCL-X(-316 to -346)	NULL		NULL	NULL	NULL	NULL	gw60_cell_98_2_181_s_112	10428030	(B) EMSA showing  Stat5 binding to  BCL-X(-316 to -346) from the human  BCL-X gene.	bind
9372	1	3850	6	11	NULL	NULL	NULL	Stat5	GP		bind					BCL-X gene	GP	human		BCL-X(-316 to -346)	NULL		NULL	NULL	NULL	NULL	gw60_cell_98_2_181_s_112	10428030	(B) EMSA showing  Stat5 binding to  BCL-X(-316 to -346) from the human  BCL-X gene.	bind
8976	1	3851	5	11	NULL	NULL	NULL	MSY2	GP		bind					Prm1	GP	wt		1-37	NULL	testis extracts	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_20_7010_s_253	11564883	(B) EMSA with testis extracts showing the binding of MSY2 and MSY4 to  Prm11-37wt but not to the mutant version used in the transgene.	bind
8977	2	3851	5	11	NULL	NULL	NULL	MSY4	GP		bind					Prm1	GP	wt		1-37	NULL	testis extracts	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_20_7010_s_253	11564883	(B) EMSA with testis extracts showing the binding of MSY2 and MSY4 to  Prm11-37wt but not to the mutant version used in the transgene.	bind
8978	3	3851	5	11	NULL	NULL	NULL	MSY2	GP		does not bind					Prm1	GP	mutant		1-37	NULL	testis extracts	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_20_7010_s_253	11564883	(B) EMSA with testis extracts showing the binding of MSY2 and MSY4 to  Prm11-37wt but not to the mutant version used in the transgene.	bind
8979	4	3851	5	11	NULL	NULL	NULL	MSY4	GP		does not bind					Prm1	GP	mutant		1-37	NULL	testis extracts	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_20_7010_s_253	11564883	(B) EMSA with testis extracts showing the binding of MSY2 and MSY4 to  Prm11-37wt but not to the mutant version used in the transgene.	bind
9373	1	3851	6	11	NULL	NULL	NULL	MSY2	GP		bind					Prm1	GP	wild type		1-37	NULL	testis extracts	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_20_7010_s_253	11564883	(B) EMSA with testis extracts showing the binding of MSY2 and MSY4 to  Prm11-37wt but not to the mutant version used in the transgene.	bind
9374	2	3851	6	11	NULL	NULL	NULL	MSY4	GP		bind					Prm1	GP	wild type		1-37	NULL	testis extracts	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_20_7010_s_253	11564883	(B) EMSA with testis extracts showing the binding of MSY2 and MSY4 to  Prm11-37wt but not to the mutant version used in the transgene.	bind
9375	3	3851	6	11	NULL	NULL	NULL	MSY2	GP		does not bind					Prm1	GP	mutant		1-37	NULL	testis extracts	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_20_7010_s_253	11564883	(B) EMSA with testis extracts showing the binding of MSY2 and MSY4 to  Prm11-37wt but not to the mutant version used in the transgene.	bind
9376	4	3851	6	11	NULL	NULL	NULL	MSY4	GP		does not bind					Prm1	GP	mutant		1-37	NULL	testis extracts	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_20_7010_s_253	11564883	(B) EMSA with testis extracts showing the binding of MSY2 and MSY4 to  Prm11-37wt but not to the mutant version used in the transgene.	bind
9111	1	3853	5	11	NULL	NULL	NULL	Galphas	GP	endogenous;; rat brain lysates	bind					GST-Hrs	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_12_5538_s_159	15469987	(B) Endogenous Galphas from rat brain lysates binds to GST-Hrs but not to GST.	bind
9112	2	3853	5	11	NULL	NULL	NULL	Galphas	GP	endogenous;; rat brain lysates	does not bind					GST	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_12_5538_s_159	15469987	(B) Endogenous Galphas from rat brain lysates binds to GST-Hrs but not to GST.	bind
9377	1	3853	6	11	NULL	NULL	NULL	Galphas	GP	endogenous;; rat brain lysates	bind					GST-Hrs	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_12_5538_s_159	15469987	(B) Endogenous Galphas from rat brain lysates binds to GST-Hrs but not to GST.	bind
9378	2	3853	6	11	NULL	NULL	NULL	Galphas	GP	endogenous;; rat brain lysates	does not bind					GST	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_12_5538_s_159	15469987	(B) Endogenous Galphas from rat brain lysates binds to GST-Hrs but not to GST.	bind
9113	1	3854	5	NULL	NULL	0	NULL	Smad7	NULL	endogenous	bind	NULL				p38	NULL	phosphorylated			NULL	in vivo	0	NULL	NULL	NULL	gw60_molbiolcell_14_2_529_s_245	12589052	(B) Endogenous Smad7 binds to phosphorylated p38 in vivo.	bind
9379	1	3854	6	NULL	NULL	0	NULL	Smad7	NULL	endogenous	bind	NULL				p38	NULL	phosphorylated			NULL	in vivo	0	NULL	NULL	NULL	gw60_molbiolcell_14_2_529_s_245	12589052	(B) Endogenous Smad7 binds to phosphorylated p38 in vivo.	bind
9114	1	3855	5	11	NULL	NULL	NULL	Nrf2	GP		bind					PSMB5	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8786_s_182	14612418	(B) Enhanced binding of Nrf2 to the  PSMB5 promoter following sulforaphane (Sul) treatment compared to that in vehicle (V)-treated  cells.	bind
9115	2	3855	5	11	NULL	NULL	NULL	Nrf2	GP		bind					PSMB5	GP			promoter	NULL	in vehicle (V)-treated cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8786_s_182	14612418	(B) Enhanced binding of Nrf2 to the  PSMB5 promoter following sulforaphane (Sul) treatment compared to that in vehicle (V)-treated  cells.	bind
9116	3	3855	5	11	NULL	NULL	NULL	Sul	Chemical	treatment with	enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8786_s_182	14612418	(B) Enhanced binding of Nrf2 to the  PSMB5 promoter following sulforaphane (Sul) treatment compared to that in vehicle (V)-treated  cells.	bind
53649	4	3855	5	11	NULL	NULL	NULL	Sul	Chemical		is					sulforaphane	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8786_s_182	14612418	(B) Enhanced binding of Nrf2 to the  PSMB5 promoter following sulforaphane (Sul) treatment compared to that in vehicle (V)-treated  cells.	bind
9380	1	3855	6	11	NULL	NULL	NULL	Nrf2	GP		bind					PSMB5	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8786_s_182	14612418	(B) Enhanced binding of Nrf2 to the  PSMB5 promoter following sulforaphane (Sul) treatment compared to that in vehicle (V)-treated  cells.	bind
9381	2	3855	6	11	NULL	NULL	NULL	statement 1	Process		occurs following					Sul	Chemical	treatment with			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8786_s_182	14612418	(B) Enhanced binding of Nrf2 to the  PSMB5 promoter following sulforaphane (Sul) treatment compared to that in vehicle (V)-treated  cells.	bind
9382	3	3855	6	11	NULL	NULL	NULL	Nrf2	GP		bind					PSMB5	GP			promoter	NULL	vehicle (V)-treated cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8786_s_182	14612418	(B) Enhanced binding of Nrf2 to the  PSMB5 promoter following sulforaphane (Sul) treatment compared to that in vehicle (V)-treated  cells.	bind
53650	4	3855	6	11	NULL	NULL	NULL	Sul	Chemical		is					sulforaphane	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8786_s_182	14612418	(B) Enhanced binding of Nrf2 to the  PSMB5 promoter following sulforaphane (Sul) treatment compared to that in vehicle (V)-treated  cells.	bind
9117	1	3856	5	11	NULL	NULL	NULL	GR	GP		bind					MMTV chromatin 	Chromosome				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_10_3255_s_73	11971959	(B) Enhancement of GR binding to MMTV chromatin by HeLa nuclear extract.	bind
9118	2	3856	5	11	NULL	NULL	NULL	HeLa nuclear extract	CellComponent		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_10_3255_s_73	11971959	(B) Enhancement of GR binding to MMTV chromatin by HeLa nuclear extract.	bind
9383	1	3856	6	11	NULL	NULL	NULL	GR	GP		bind					MMTV chromatin	Chromosome				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_10_3255_s_73	11971959	(B) Enhancement of GR binding to MMTV chromatin by HeLa nuclear extract.	bind
9384	2	3856	6	11	NULL	NULL	NULL	HeLa nuclear extract	CellComponent		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_10_3255_s_73	11971959	(B) Enhancement of GR binding to MMTV chromatin by HeLa nuclear extract.	bind
9119	1	3857	5	11	NULL	NULL	NULL	Ephrin-B1-Fc	GP		bind		specifically			neural crest cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_8_571_s_159	9259560	(b) Ephrin-B1-Fc bound specifically to neural crest cells, indicating that receptor expression was maintained  in vitro.	bind
9120	2	3857	5	11	NULL	NULL	NULL	statement 1	Process		indicate					maintained receptor expression 	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_currbiol_7_8_571_s_159	9259560	(b) Ephrin-B1-Fc bound specifically to neural crest cells, indicating that receptor expression was maintained  in vitro.	bind
9385	1	3857	6	11	NULL	NULL	NULL	Ephrin-B1-Fc	GP		bind		specifically			neural crest cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_8_571_s_159	9259560	(b) Ephrin-B1-Fc bound specifically to neural crest cells, indicating that receptor expression was maintained  in vitro.	bind
11651	2	3857	6	11	NULL	NULL	NULL	statement 1	Process		indicates					maintained receptor expression	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_currbiol_7_8_571_s_159	9259560	(b) Ephrin-B1-Fc bound specifically to neural crest cells, indicating that receptor expression was maintained  in vitro.	bind
9121	1	3860	5	11	NULL	NULL	NULL	P6EtG/HLA-A2	GP		bind					A6	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_13_4_475_s_110	11070166	(B) Equilibrium binding data for P6EtG/HLA-A2 binding to A6.	bind
9387	1	3860	6	11	NULL	NULL	NULL	P6EtG/HLA-A2	GP		bind					A6	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_13_4_475_s_110	11070166	(B) Equilibrium binding data for P6EtG/HLA-A2 binding to A6.	bind
9447	1	3861	5	11	NULL	NULL	NULL	ER	Chemical		does not bind					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_166_1_97_s_157	15240572	(B) ER and LG3 do not bind to an analytical heparin-agarose column.	bind
9448	2	3861	5	11	NULL	NULL	NULL	LG3	GP		does not bind					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_166_1_97_s_157	15240572	(B) ER and LG3 do not bind to an analytical heparin-agarose column.	bind
9388	1	3861	6	11	NULL	NULL	NULL	ER	Chemical		does not bind					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_166_1_97_s_157	15240572	(B) ER and LG3 do not bind to an analytical heparin-agarose column.	bind
9389	2	3861	6	11	NULL	NULL	NULL	LG3	GP		does not bind					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_166_1_97_s_157	15240572	(B) ER and LG3 do not bind to an analytical heparin-agarose column.	bind
9122	1	3862	5	11	NULL	NULL	NULL	ER-E2F3	GP		bind							E2F-responsive		promoters	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_7_2660_s_209	15767672	(B) ER-E2F3 binds to E2F-responsive promoters  and recruits pRB upon activation.	bind
9123	2	3862	5	11	NULL	NULL	NULL	ER-E2F3	GP	activated	recruit					pRB	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_7_2660_s_209	15767672	(B) ER-E2F3 binds to E2F-responsive promoters  and recruits pRB upon activation.	bind
9390	1	3862	6	11	NULL	NULL	NULL	ER-E2F3	GP		bind							E2F responsive		promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_7_2660_s_209	15767672	(B) ER-E2F3 binds to E2F-responsive promoters  and recruits pRB upon activation.	bind
9391	2	3862	6	11	NULL	NULL	NULL	ER-E2F3	GP	activated	recruits					pRB	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_7_2660_s_209	15767672	(B) ER-E2F3 binds to E2F-responsive promoters  and recruits pRB upon activation.	bind
9125	1	3863	5	11	NULL	NULL	NULL	ERalpha	GP		bind					hTERT	GP			ERE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_11_3764_s_83	10805720	(b) ERalpha binding to the hTERT ERE.	bind
9392	1	3863	6	11	NULL	NULL	NULL	ERalpha	GP		bind					hTERT	GP			ERE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_11_3764_s_83	10805720	(b) ERalpha binding to the hTERT ERE.	bind
9126	1	3864	5	10	NULL	0	NULL	ERKs	NULL		does not bind	NULL				Mxi2	NULL	mutant	 WI		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_9_3079_s_299	12697810	(B) ERKs cannot bind to the Mxi2 WI mutant form.	bind
9393	1	3864	6	11	NULL	NULL	NULL	ERK	GP		does not bind					Mxi2	GP	mutant	WI		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_9_3079_s_299	12697810	(B) ERKs cannot bind to the Mxi2 WI mutant form.	bind
9127	1	3865	5	11	NULL	NULL	NULL	ETO-2	GP		bind					HDAC1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6470_s_172	11533236	(B) ETO-2 binds HDACs 1, 2, 3, 6, and 8.	bind
9128	2	3865	5	11	NULL	NULL	NULL	ETO-2	GP		bind					HDAC2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6470_s_172	11533236	(B) ETO-2 binds HDACs 1, 2, 3, 6, and 8.	bind
9129	3	3865	5	11	NULL	NULL	NULL	ETO-2	GP		bind					HDAC3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6470_s_172	11533236	(B) ETO-2 binds HDACs 1, 2, 3, 6, and 8.	bind
9130	4	3865	5	11	NULL	NULL	NULL	ETO-2	GP		bind					HDAC6	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6470_s_172	11533236	(B) ETO-2 binds HDACs 1, 2, 3, 6, and 8.	bind
9131	5	3865	5	11	NULL	NULL	NULL	ETO-2	GP		bind					HDAC8	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6470_s_172	11533236	(B) ETO-2 binds HDACs 1, 2, 3, 6, and 8.	bind
9394	1	3865	6	11	NULL	NULL	NULL	ETO-2	GP		bind					HDAC1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6470_s_172	11533236	(B) ETO-2 binds HDACs 1, 2, 3, 6, and 8.	bind
9395	2	3865	6	11	NULL	NULL	NULL	ETO-2	GP		bind					HDAC2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6470_s_172	11533236	(B) ETO-2 binds HDACs 1, 2, 3, 6, and 8.	bind
9396	3	3865	6	11	NULL	NULL	NULL	ETO-2	GP		bind					HDAC3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6470_s_172	11533236	(B) ETO-2 binds HDACs 1, 2, 3, 6, and 8.	bind
9397	4	3865	6	11	NULL	NULL	NULL	ETO-2	GP		bind					HDAC6	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6470_s_172	11533236	(B) ETO-2 binds HDACs 1, 2, 3, 6, and 8.	bind
9398	5	3865	6	11	NULL	NULL	NULL	ETO-2	GP		bind					HDAC8	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6470_s_172	11533236	(B) ETO-2 binds HDACs 1, 2, 3, 6, and 8.	bind
9442	1	3866	5	11	NULL	NULL	NULL	MyoD	GP		direct					MyHC 	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6600_s_196	10938134	(B) Even though cain cotransfection blocks MyoD-directed MyHC expression, these cells still express myogenin, suggesting no loss of transfected cells or in their respecification to the myogenic lineage.	bind
9443	2	3866	5	11	NULL	NULL	NULL	cain	GP	transfection	blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6600_s_196	10938134	(B) Even though cain cotransfection blocks MyoD-directed MyHC expression, these cells still express myogenin, suggesting no loss of transfected cells or in their respecification to the myogenic lineage.	bind
9444	3	3866	5	11	NULL	NULL	NULL	cells	cell		express					myogenin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6600_s_196	10938134	(B) Even though cain cotransfection blocks MyoD-directed MyHC expression, these cells still express myogenin, suggesting no loss of transfected cells or in their respecification to the myogenic lineage.	bind
9445	4	3866	5	11	NULL	NULL	NULL	statement 3	Process		suggest					 transfected cells	Cell	 no loss of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6600_s_196	10938134	(B) Even though cain cotransfection blocks MyoD-directed MyHC expression, these cells still express myogenin, suggesting no loss of transfected cells or in their respecification to the myogenic lineage.	bind
9446	5	3866	5	11	NULL	NULL	NULL	statement 3	Process		suggest					myogenic lineage	Cell	respecification to			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6600_s_196	10938134	(B) Even though cain cotransfection blocks MyoD-directed MyHC expression, these cells still express myogenin, suggesting no loss of transfected cells or in their respecification to the myogenic lineage.	bind
9670	1	3866	6	11	NULL	NULL	NULL	MyoD-	GP		directs					MyHC	GP	expression of 			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6600_s_196	10938134	(B) Even though cain cotransfection blocks MyoD-directed MyHC expression, these cells still express myogenin, suggesting no loss of transfected cells or in their respecification to the myogenic lineage.	bind
9671	2	3866	6	11	NULL	NULL	NULL	cain	GP		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6600_s_196	10938134	(B) Even though cain cotransfection blocks MyoD-directed MyHC expression, these cells still express myogenin, suggesting no loss of transfected cells or in their respecification to the myogenic lineage.	bind
9132	1	3868	5	11	NULL	NULL	NULL	Exip	GP		bind					IRAK	GP				NULL		NULL	NULL	NULL	NULL	gw70_febslett_575_1_136_s_124	15388348	(B) Exip binds to IRAK.	bind
9399	1	3868	6	11	NULL	NULL	NULL	Exip	GP		bind					IRAK	GP				NULL		NULL	NULL	NULL	NULL	gw70_febslett_575_1_136_s_124	15388348	(B) Exip binds to IRAK.	bind
9133	1	3869	5	11	NULL	NULL	NULL	Exip	GP		bind					Tollip	GP				NULL		NULL	NULL	NULL	NULL	gw70_febslett_575_1_136_s_111	15388348	(B) Exip binds to Tollip irrespective to IL-1  stimulation.	bind
9134	2	3869	5	11	NULL	NULL	NULL	statement 1	Process		irrespective to					IL-1	GP	stimulation of			NULL		NULL	NULL	NULL	NULL	gw70_febslett_575_1_136_s_111	15388348	(B) Exip binds to Tollip irrespective to IL-1  stimulation.	bind
9400	1	3869	6	11	NULL	NULL	NULL	Exip	GP		bind					Tollip	GP				NULL		NULL	NULL	NULL	NULL	gw70_febslett_575_1_136_s_111	15388348	(B) Exip binds to Tollip irrespective to IL-1  stimulation.	bind
11652	2	3869	6	11	NULL	NULL	NULL	statement 1	GP		irrespective to					IL-1	GP	stimulation of 			NULL		NULL	NULL	NULL	NULL	gw70_febslett_575_1_136_s_111	15388348	(B) Exip binds to Tollip irrespective to IL-1  stimulation.	bind
9135	1	3870	5	11	NULL	NULL	NULL	NGFI-B/RXR	GP		bind					DR1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_6_849_s_260	9660968	(B) Expected role of NGFI-B's 5  flanking sequence in NGFI-B/RXR binding to DR1-DR5.	bind
9136	2	3870	5	11	NULL	NULL	NULL	NGFI-B/RXR	GP		bind					DR2	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_6_849_s_260	9660968	(B) Expected role of NGFI-B's 5  flanking sequence in NGFI-B/RXR binding to DR1-DR5.	bind
9137	3	3870	5	11	NULL	NULL	NULL	NGFI-B/RXR	GP		bind					DR3	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_6_849_s_260	9660968	(B) Expected role of NGFI-B's 5  flanking sequence in NGFI-B/RXR binding to DR1-DR5.	bind
9138	4	3870	5	11	NULL	NULL	NULL	NGFI-B/RXR	GP		bind					DR4	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_6_849_s_260	9660968	(B) Expected role of NGFI-B's 5  flanking sequence in NGFI-B/RXR binding to DR1-DR5.	bind
9139	5	3870	5	11	NULL	NULL	NULL	NGFI-B/RXR	GP		bind					DR5	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_6_849_s_260	9660968	(B) Expected role of NGFI-B's 5  flanking sequence in NGFI-B/RXR binding to DR1-DR5.	bind
9401	1	3870	6	11	NULL	NULL	NULL	NGFI-B/RXR	GP		bind					DR1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_6_849_s_260	9660968	(B) Expected role of NGFI-B's 5  flanking sequence in NGFI-B/RXR binding to DR1-DR5.	bind
44775	2	3870	6	11	NULL	NULL	NULL	NGFI-B/RXR	GP		bind					DR2	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_6_849_s_260	9660968	(B) Expected role of NGFI-B's 5  flanking sequence in NGFI-B/RXR binding to DR1-DR5.	bind
44776	3	3870	6	11	NULL	NULL	NULL	NGFI-B/RXR	GP		bind					DR3	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_6_849_s_260	9660968	(B) Expected role of NGFI-B's 5  flanking sequence in NGFI-B/RXR binding to DR1-DR5.	bind
44777	4	3870	6	11	NULL	NULL	NULL	NGFI-B/RXR	GP		bind					DR4	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_6_849_s_260	9660968	(B) Expected role of NGFI-B's 5  flanking sequence in NGFI-B/RXR binding to DR1-DR5.	bind
44778	5	3870	6	11	NULL	NULL	NULL	NGFI-B/RXR	GP		bind					DR5	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_6_849_s_260	9660968	(B) Expected role of NGFI-B's 5  flanking sequence in NGFI-B/RXR binding to DR1-DR5.	bind
9140	1	3871	5	11	NULL	NULL	NULL	AKAP79	GP	wt	bind					RII	GP				NULL	in stable cells	NULL	NULL	NULL	NULL	gw60_neuron_19_1_185_s_51	9247274	(B) Expression and RII binding properties of AKAP79wt and AKAP79pro in the stable cells.	bind
9141	2	3871	5	11	NULL	NULL	NULL	AKAP79	GP	pro	bind					RII	GP				NULL	in stable cells	NULL	NULL	NULL	NULL	gw60_neuron_19_1_185_s_51	9247274	(B) Expression and RII binding properties of AKAP79wt and AKAP79pro in the stable cells.	bind
9402	1	3871	6	11	NULL	NULL	NULL	AKAP79	GP	wild type	bind					RII	GP				NULL	stable cells	NULL	NULL	NULL	NULL	gw60_neuron_19_1_185_s_51	9247274	(B) Expression and RII binding properties of AKAP79wt and AKAP79pro in the stable cells.	bind
9403	2	3871	6	11	NULL	NULL	NULL	AKAP79	GP	pro	bind					RII	GP				NULL	stable cells	NULL	NULL	NULL	NULL	gw60_neuron_19_1_185_s_51	9247274	(B) Expression and RII binding properties of AKAP79wt and AKAP79pro in the stable cells.	bind
9211	1	3873	5	11	NULL	NULL	NULL	GRIP1	GP		bind		specifically			liprin-4	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_neuron_34_1_39_s_45	11931740	(B) Filter overlay assay showing specific in vitro binding between GRIP1 and liprin- 4.	bind
9404	1	3873	6	11	NULL	NULL	NULL	GRIP1	GP		bind		specifically			liprin-4	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_neuron_34_1_39_s_45	11931740	(B) Filter overlay assay showing specific in vitro binding between GRIP1 and liprin- 4.	bind
9212	1	3874	5	11	NULL	NULL	NULL	Fli1	GP		bind					SCL	GP			+19 core enhancer	NULL	in blood cell lines	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_7_2615_s_203	16537906	(B) Fli1, Elf1, and GATA2 bind the SCL +19 core enhancer in  both blood and bone cell lines.	bind
9213	2	3874	5	11	NULL	NULL	NULL	Fli1	GP		bind					SCL	GP			+19 core enhancer	NULL	in bone cell lines	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_7_2615_s_203	16537906	(B) Fli1, Elf1, and GATA2 bind the SCL +19 core enhancer in  both blood and bone cell lines.	bind
9215	4	3874	5	11	NULL	NULL	NULL	Elf1	GP		bind					SCL	GP			+19 core enhancer	NULL	in bone cell lines	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_7_2615_s_203	16537906	(B) Fli1, Elf1, and GATA2 bind the SCL +19 core enhancer in  both blood and bone cell lines.	bind
9216	5	3874	5	11	NULL	NULL	NULL	GATA2	GP		bind					SCL	GP			+19 core enhancer	NULL	in blood cell lines	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_7_2615_s_203	16537906	(B) Fli1, Elf1, and GATA2 bind the SCL +19 core enhancer in  both blood and bone cell lines.	bind
9217	6	3874	5	11	NULL	NULL	NULL	GATA2	GP		bind					SCL	GP			+19 core enhancer	NULL	in bone cell lines	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_7_2615_s_203	16537906	(B) Fli1, Elf1, and GATA2 bind the SCL +19 core enhancer in  both blood and bone cell lines.	bind
9405	1	3874	6	11	NULL	NULL	NULL	Fli1	GP		bind					SCL	GP			+19 core enhancer	NULL	blood cell lines	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_7_2615_s_203	16537906	(B) Fli1, Elf1, and GATA2 bind the SCL +19 core enhancer in  both blood and bone cell lines.	bind
9406	2	3874	6	11	NULL	NULL	NULL	Elf1	GP		bind					SCL 	GP			+19 core enhancer	NULL	blood cell lines	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_7_2615_s_203	16537906	(B) Fli1, Elf1, and GATA2 bind the SCL +19 core enhancer in  both blood and bone cell lines.	bind
9407	3	3874	6	11	NULL	NULL	NULL	GATA2	GP		bind					SCL 	GP			+19 core enhancer	NULL	blood cell lines	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_7_2615_s_203	16537906	(B) Fli1, Elf1, and GATA2 bind the SCL +19 core enhancer in  both blood and bone cell lines.	bind
11653	4	3874	6	11	NULL	NULL	NULL	Fli1	GP		bind					SCL	GP			+19 core enhancer	NULL	bone cell line	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_7_2615_s_203	16537906	(B) Fli1, Elf1, and GATA2 bind the SCL +19 core enhancer in  both blood and bone cell lines.	bind
11654	5	3874	6	11	NULL	NULL	NULL	Elf1	GP		bind					SCL	GP			+19 core enhancer	NULL	bone cell line	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_7_2615_s_203	16537906	(B) Fli1, Elf1, and GATA2 bind the SCL +19 core enhancer in  both blood and bone cell lines.	bind
11655	6	3874	6	11	NULL	NULL	NULL	GATA-2	GP		bind					SCL	GP			+19 core enhancer	NULL	bone cell line	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_7_2615_s_203	16537906	(B) Fli1, Elf1, and GATA2 bind the SCL +19 core enhancer in  both blood and bone cell lines.	bind
9218	1	3875	5	11	NULL	NULL	NULL	BLyS	GP		bind					 B cells	Cell	splenic			NULL		NULL	NULL	NULL	NULL	gw60_immunity_14_5_573_s_108	11371359	(B) Flow cytometric analysis of BLyS binding to splenic B cells.	bind
9408	1	3875	6	11	NULL	NULL	NULL	BLyS	GP		bind					B cells	Cell	splenic			NULL		NULL	NULL	NULL	NULL	gw60_immunity_14_5_573_s_108	11371359	(B) Flow cytometric analysis of BLyS binding to splenic B cells.	bind
9214	3	3876	5	11	NULL	NULL	NULL	Elf1	GP		bind					SCL	GP			+19 core enhancer	NULL	in blood cell lines	NULL	NULL	NULL	NULL	gw60_neuron_37_4_555_s_36	12597853	(B) FMRP binds to CYFIP, which interacts directly with F-actin.	bind
9219	1	3876	5	11	NULL	NULL	NULL	FMRP	GP		bind					CYFIP	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_37_4_555_s_36	12597853	(B) FMRP binds to CYFIP, which interacts directly with F-actin.	bind
9220	2	3876	5	11	NULL	NULL	NULL	CYFIP	GP		interact with		directly			F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_37_4_555_s_36	12597853	(B) FMRP binds to CYFIP, which interacts directly with F-actin.	bind
9409	1	3876	6	11	NULL	NULL	NULL	FMRP	GP		bind					CYFIP	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_37_4_555_s_36	12597853	(B) FMRP binds to CYFIP, which interacts directly with F-actin.	bind
9410	2	3876	6	11	NULL	NULL	NULL	CYFIP	GP		interacts		directly			F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_37_4_555_s_36	12597853	(B) FMRP binds to CYFIP, which interacts directly with F-actin.	bind
9221	1	3877	5	11	NULL	NULL	NULL	xUBF	GP		bind							Xenopus		core promoter region	NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_5_1059_s_160	11106745	(B) Footprint analysis of xUBF bound to the  Xenopus core promoter region.	bind
9411	1	3877	6	11	NULL	NULL	NULL	xUBF	GP		bind							Xenopus 		core promoter region	NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_5_1059_s_160	11106745	(B) Footprint analysis of xUBF bound to the  Xenopus core promoter region.	bind
9222	1	3878	5	11	NULL	NULL	NULL	Mpc54p-GFP components	GP		bind					SPBs	CellComponent				NULL	in wild-type cells in meiosis II	NULL	NULL	NULL	NULL	gw70_cellbiol_171_4_627_s_148	16286509	(B) FRAP analysis of the binding of Mpc54p-GFP components to SPBs in wild-type cells  in meiosis II.	bind
9412	1	3878	6	11	NULL	NULL	NULL	Mpc54p-GFP	GP		bind					SPBs	CellComponent				NULL	wild-type cells in meiosis II	NULL	NULL	NULL	NULL	gw70_cellbiol_171_4_627_s_148	16286509	(B) FRAP analysis of the binding of Mpc54p-GFP components to SPBs in wild-type cells  in meiosis II.	bind
9223	1	3879	5	11	NULL	NULL	NULL	FRS2alpha	GP		bind					TrkA	GP	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_3_979_s_238	10629055	(B) FRS2alpha binds to tyrosine-phosphorylated TrkA.	bind
9413	1	3879	6	11	NULL	NULL	NULL	FRS2alpha	GP		bind					TrkA	GP	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_3_979_s_238	10629055	(B) FRS2alpha binds to tyrosine-phosphorylated TrkA.	bind
9224	1	3880	5	11	NULL	NULL	NULL	GFP-Crz1p		full-length	bind		constitutively	S409		importin Nmd5p	GP				NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_3_5_1147_s_197	15470242	(B) Full-length GFP-Crz1pS409,410,423A constitutively binds the importin Nmd5p.	bind
9225	2	3880	5	11	NULL	NULL	NULL	GFP-Crz1p	GP	full-length	bind		constitutively	S410		importin Nmd5p	GP				NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_3_5_1147_s_197	15470242	(B) Full-length GFP-Crz1pS409,410,423A constitutively binds the importin Nmd5p.	bind
9226	3	3880	5	11	NULL	NULL	NULL	GFP-Crz1p	GP	full-length	bind		constitutively	S423A		importin Nmd5p	GP				NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_3_5_1147_s_197	15470242	(B) Full-length GFP-Crz1pS409,410,423A constitutively binds the importin Nmd5p.	bind
9417	1	3880	6	11	NULL	NULL	NULL	GFP-Crz1p	GP	full length	bind		constitutively	S409		importin Nmd5p	GP				NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_3_5_1147_s_197	15470242	(B) Full-length GFP-Crz1pS409,410,423A constitutively binds the importin Nmd5p.	bind
9418	2	3880	6	11	NULL	NULL	NULL	GFP-Crz1p	GP	full length	bind		constitutively	S410		importin Nmd5p	GP				NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_3_5_1147_s_197	15470242	(B) Full-length GFP-Crz1pS409,410,423A constitutively binds the importin Nmd5p.	bind
9419	3	3880	6	11	NULL	NULL	NULL	GFP-Crz1p	GP	full length	bind		constitutively	S423A		importin Nmd5p	GP				NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_3_5_1147_s_197	15470242	(B) Full-length GFP-Crz1pS409,410,423A constitutively binds the importin Nmd5p.	bind
9227	1	3882	5	11	NULL	NULL	NULL	FUS3	GP		bind					At2S3	GP			RY-G-box complex in promoter	NULL		NULL	NULL	NULL	NULL	gw70_development_130_24_6065_s_100	14597573	(B) FUS3 and LEC2 bind to the  RY-G-box complex in the  At2S3 promoter.	bind
9228	2	3882	5	11	NULL	NULL	NULL	LEC2	GP		bind					At2S3	GP			RY-G-box complex in promoter	NULL		NULL	NULL	NULL	NULL	gw70_development_130_24_6065_s_100	14597573	(B) FUS3 and LEC2 bind to the  RY-G-box complex in the  At2S3 promoter.	bind
9420	1	3882	6	11	NULL	NULL	NULL	FUS3	GP		bind					At2S3	GP			RY-G-box complex of the promoter	NULL		NULL	NULL	NULL	NULL	gw70_development_130_24_6065_s_100	14597573	(B) FUS3 and LEC2 bind to the  RY-G-box complex in the  At2S3 promoter.	bind
9421	2	3882	6	11	NULL	NULL	NULL	LEC2	GP		bind					At2S3	GP			RY-G-box complex of the promoter	NULL		NULL	NULL	NULL	NULL	gw70_development_130_24_6065_s_100	14597573	(B) FUS3 and LEC2 bind to the  RY-G-box complex in the  At2S3 promoter.	bind
9229	1	3883	5	11	NULL	NULL	NULL	Gads/Grb2	GP		bind					SLP-76	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_7_2515_s_241	12640133	(B) Gab2 competes for  Gads/Grb2 binding with SLP-76.	bind
9230	2	3883	5	11	NULL	NULL	NULL	Gab2	GP		bind					SLP-76	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_7_2515_s_241	12640133	(B) Gab2 competes for  Gads/Grb2 binding with SLP-76.	bind
9231	3	3883	5	11	NULL	NULL	NULL	statement 2	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_7_2515_s_241	12640133	(B) Gab2 competes for  Gads/Grb2 binding with SLP-76.	bind
9625	1	3883	6	11	NULL	NULL	NULL	Gads/Grb2	GP		bind					SLP-76	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_7_2515_s_241	12640133	(B) Gab2 competes for  Gads/Grb2 binding with SLP-76.	bind
9626	2	3883	6	11	NULL	NULL	NULL	Gab2	GP		bind					SLP-76	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_7_2515_s_241	12640133	(B) Gab2 competes for  Gads/Grb2 binding with SLP-76.	bind
9627	3	3883	6	11	NULL	NULL	NULL	statement 1	Process		competes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_7_2515_s_241	12640133	(B) Gab2 competes for  Gads/Grb2 binding with SLP-76.	bind
9232	1	3884	5	11	NULL	NULL	NULL	Gads/Grb2	GP		bind					SLP-76	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_7_2515_s_241	12640133	(B) Gab2 competes for Gads/Grb2 binding with SLP-76.	bind
9233	2	3884	5	11	NULL	NULL	NULL	Gab2	GP		bind					SLP-76	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_7_2515_s_241	12640133	(B) Gab2 competes for Gads/Grb2 binding with SLP-76.	bind
9234	3	3884	5	11	NULL	NULL	NULL	statement 2	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_7_2515_s_241	12640133	(B) Gab2 competes for Gads/Grb2 binding with SLP-76.	bind
9659	1	3884	6	11	NULL	NULL	NULL	Gads/Grb2	GP		bind					SLP-76	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_7_2515_s_241	12640133	(B) Gab2 competes for Gads/Grb2 binding with SLP-76.	bind
9660	2	3884	6	11	NULL	NULL	NULL	Gab2	GP		bind					SLP-76	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_7_2515_s_241	12640133	(B) Gab2 competes for Gads/Grb2 binding with SLP-76.	bind
9661	3	3884	6	11	NULL	NULL	NULL	statement 1	Process		competes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_7_2515_s_241	12640133	(B) Gab2 competes for Gads/Grb2 binding with SLP-76.	bind
9235	1	3885	5	11	NULL	NULL	NULL	trypomastigote	Organism	T. cruzi	bind					CASM cells	Cell	human			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_11_6717_s_47	15501810	(B) Galectin-3 enhances  T. cruzi trypomastigote binding to human CASM cells.	bind
9236	2	3885	5	11	NULL	NULL	NULL	Galectin-3	GP		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_11_6717_s_47	15501810	(B) Galectin-3 enhances  T. cruzi trypomastigote binding to human CASM cells.	bind
9422	1	3885	6	11	NULL	NULL	NULL	trypomastigote	Organism	T. cruzi	bind					CASM cells	Cell	human			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_11_6717_s_47	15501810	(B) Galectin-3 enhances  T. cruzi trypomastigote binding to human CASM cells.	bind
9423	2	3885	6	11	NULL	NULL	NULL	Galectin-3	GP		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_11_6717_s_47	15501810	(B) Galectin-3 enhances  T. cruzi trypomastigote binding to human CASM cells.	bind
9237	1	3886	5	11	NULL	NULL	NULL	GATA-1	GP		bind					GGE probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_2_713_s_212	10611250	(B) GATA-1, GATA-2, and GATA-3 can bind to the GGE probe.	bind
9238	2	3886	5	11	NULL	NULL	NULL	GATA-2	GP		bind					GGE probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_2_713_s_212	10611250	(B) GATA-1, GATA-2, and GATA-3 can bind to the GGE probe.	bind
9239	3	3886	5	11	NULL	NULL	NULL	GATA-3	GP		bind					GGE probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_2_713_s_212	10611250	(B) GATA-1, GATA-2, and GATA-3 can bind to the GGE probe.	bind
9424	1	3886	6	11	NULL	NULL	NULL	GATA-1	GP		bind					GGE probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_2_713_s_212	10611250	(B) GATA-1, GATA-2, and GATA-3 can bind to the GGE probe.	bind
9425	2	3886	6	11	NULL	NULL	NULL	GATA-2	GP		bind					GGE probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_2_713_s_212	10611250	(B) GATA-1, GATA-2, and GATA-3 can bind to the GGE probe.	bind
9426	3	3886	6	11	NULL	NULL	NULL	GATA-3	GP		bind					GGE probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_2_713_s_212	10611250	(B) GATA-1, GATA-2, and GATA-3 can bind to the GGE probe.	bind
9240	2	3887	5	11	NULL	NULL	NULL	Gcn4	GP		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_7_2078_s_390	11884596	(B) Gcn4 binds to Ty1 sequences harboring Gcn4 binding sites.	bind
53651	1	3887	5	11	NULL	NULL	NULL	Ty1 sequences	GP		harbor								Gcn4 binding sites		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_7_2078_s_390	11884596	(B) Gcn4 binds to Ty1 sequences harboring Gcn4 binding sites.	bind
9427	1	3887	6	11	NULL	NULL	NULL	Ty1 sequences	GP		harbor								Gcn4 binding sites		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_7_2078_s_390	11884596	(B) Gcn4 binds to Ty1 sequences harboring Gcn4 binding sites.	bind
9428	2	3887	6	11	NULL	NULL	NULL	Gcn4	GP		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_7_2078_s_390	11884596	(B) Gcn4 binds to Ty1 sequences harboring Gcn4 binding sites.	bind
9596	1	3888	5	11	NULL	NULL	NULL	3H-IP6	Chemical		bind					DNA-PK	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_102_6_721_s_151	11030616	(B) Gel  filtration analyses of 3H-IP6 binding by DNA-PK.	bind
9429	1	3888	6	11	NULL	NULL	NULL	3H-IP6	Chemical		bind					DNA-PK	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_102_6_721_s_151	11030616	(B) Gel  filtration analyses of 3H-IP6 binding by DNA-PK.	bind
9597	1	3889	5	11	NULL	NULL	NULL	SoxS	GP		bind					yggX	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_22_6624_s_139	14594836	(B) Gel mobility shift assay of SoxS binding to the  yggX promoter.	bind
9430	1	3889	6	11	NULL	NULL	NULL	SoxS	GP		bind					yggX	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_22_6624_s_139	14594836	(B) Gel mobility shift assay of SoxS binding to the  yggX promoter.	bind
9598	1	3890	5	11	NULL	NULL	NULL	PirR	GP		bind					pirAB- pirR	GP			intergenic region	NULL		NULL	NULL	NULL	NULL	gw70_febslett_574_1_101_s_155	15358547	(B) Gel mobility shift assays of PirR binding to  the  pirAB- pirR intergenic region.	bind
9431	1	3890	6	11	NULL	NULL	NULL	PirR	GP		bind					pirAB- pirR	GP			intergenic region	NULL		NULL	NULL	NULL	NULL	gw70_febslett_574_1_101_s_155	15358547	(B) Gel mobility shift assays of PirR binding to  the  pirAB- pirR intergenic region.	bind
9601	1	3891	5	11	NULL	NULL	NULL	primary pro-B cells proteins	GP		bind									E i NF- B site	NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_2_131_s_146	9047235	(B) Gel mobility supershift analysis of primary pro- and pre-B cell proteins binding to the E i NF- B site.	bind
9602	2	3891	5	11	NULL	NULL	NULL	primary pre-B cells proteins	GP		bind									E i NF- B site	NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_2_131_s_146	9047235	(B) Gel mobility supershift analysis of primary pro- and pre-B cell proteins binding to the E i NF- B site.	bind
9432	1	3891	6	11	NULL	NULL	NULL	primary pro-B cell proteins	GP		bind									E i NF- B site	NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_2_131_s_146	9047235	(B) Gel mobility supershift analysis of primary pro- and pre-B cell proteins binding to the E i NF- B site.	bind
9433	2	3891	6	11	NULL	NULL	NULL	primary pre-B cell proteins	GP		bind 									E i NF- B site	NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_2_131_s_146	9047235	(B) Gel mobility supershift analysis of primary pro- and pre-B cell proteins binding to the E i NF- B site.	bind
9603	1	3893	5	11	NULL	NULL	NULL				bind			POU domain		DNA fragment	NucleicAcid			promoter 	NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_2_397_s_153	12191484	(B) Gel shift analysis of POU domain (POU*) and TBP binding to promoter DNA fragment.	bind
9604	2	3893	5	11	NULL	NULL	NULL	TBP	GP		bind					DNA fragment	NucleicAcid			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_2_397_s_153	12191484	(B) Gel shift analysis of POU domain (POU*) and TBP binding to promoter DNA fragment.	bind
9434	1	3893	6	11	NULL	NULL	NULL				bind			POU domain		DNA fragment	NucleicAcid			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_2_397_s_153	12191484	(B) Gel shift analysis of POU domain (POU*) and TBP binding to promoter DNA fragment.	bind
9435	2	3893	6	11	NULL	NULL	NULL	TBP	GP		bind					DNA fragment	NucleicAcid			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_2_397_s_153	12191484	(B) Gel shift analysis of POU domain (POU*) and TBP binding to promoter DNA fragment.	bind
9605	1	3894	5	11	NULL	NULL	NULL	LuxR	GP		bind					luxI DNA	NucleicAcid			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_3_631_s_87	14729687	(B) Gel shift assay of LuxR binding to  luxI promoter DNA.	bind
9436	1	3894	6	11	NULL	NULL	NULL	LuxR	GP		bind					luxI DNA	NucleicAcid			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_3_631_s_87	14729687	(B) Gel shift assay of LuxR binding to  luxI promoter DNA.	bind
9599	1	3896	5	11	NULL	NULL	NULL	Tem1	GP		bind					Bfa1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_219_s_177	14734533	(B) Gic1  can disrupt binding of Tem1 to Bfa1.	bind
9600	2	3896	5	11	NULL	NULL	NULL	Gic1	GP		disrupt					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_219_s_177	14734533	(B) Gic1  can disrupt binding of Tem1 to Bfa1.	bind
9437	1	3896	6	11	NULL	NULL	NULL	Tem1	GP		bind					Bfa1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_219_s_177	14734533	(B) Gic1  can disrupt binding of Tem1 to Bfa1.	bind
9438	2	3896	6	11	NULL	NULL	NULL	Gic1	GP		disrupts					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_219_s_177	14734533	(B) Gic1  can disrupt binding of Tem1 to Bfa1.	bind
9606	1	3897	5	11	NULL	NULL	NULL	Gic1	GP		bind		directly			Bfa1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_219_s_142	14734533	(B) Gic1 binds directly  to Bfa1, Bub2, Tem1, and Cdc14.	bind
9607	2	3897	5	11	NULL	NULL	NULL	Gic1	GP		bind		directly			Bub2	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_219_s_142	14734533	(B) Gic1 binds directly  to Bfa1, Bub2, Tem1, and Cdc14.	bind
9608	3	3897	5	11	NULL	NULL	NULL	Gic1	GP		bind		directly			Tem1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_219_s_142	14734533	(B) Gic1 binds directly  to Bfa1, Bub2, Tem1, and Cdc14.	bind
9609	4	3897	5	11	NULL	NULL	NULL	Gic1	GP		bind		directly			Cdc14	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_219_s_142	14734533	(B) Gic1 binds directly  to Bfa1, Bub2, Tem1, and Cdc14.	bind
9449	1	3897	6	11	NULL	NULL	NULL	Gic1	GP		bind		directly			Bfa1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_219_s_142	14734533	(B) Gic1 binds directly  to Bfa1, Bub2, Tem1, and Cdc14.	bind
9450	2	3897	6	11	NULL	NULL	NULL	Gic1	GP		bind		directly			Bub2	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_219_s_142	14734533	(B) Gic1 binds directly  to Bfa1, Bub2, Tem1, and Cdc14.	bind
9451	3	3897	6	11	NULL	NULL	NULL	Gic1	GP		bind		directly			Tem1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_219_s_142	14734533	(B) Gic1 binds directly  to Bfa1, Bub2, Tem1, and Cdc14.	bind
9452	4	3897	6	11	NULL	NULL	NULL	Gic1	GP		bind		directly			Cdc14	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_219_s_142	14734533	(B) Gic1 binds directly  to Bfa1, Bub2, Tem1, and Cdc14.	bind
9610	1	3898	5	11	NULL	NULL	NULL	GIPC	GP		bind			L142A		TrkA	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_3_615_s_219	11251075	(B) GIPC(L142A/G143E) binds TrkA.	bind
9611	2	3898	5	11	NULL	NULL	NULL	GIPC	GP		bind			G143E		TrkA	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_3_615_s_219	11251075	(B) GIPC(L142A/G143E) binds TrkA.	bind
9453	1	3898	6	11	NULL	NULL	NULL	GIPC	GP		bind			L142A		TrkA	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_3_615_s_219	11251075	(B) GIPC(L142A/G143E) binds TrkA.	bind
9454	2	3898	6	11	NULL	NULL	NULL	GIPC	GP		bind			G143E		TrkA	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_3_615_s_219	11251075	(B) GIPC(L142A/G143E) binds TrkA.	bind
9612	1	3899	5	11	NULL	NULL	NULL	GLD-1	GP		bind									GRE	NULL		NULL	NULL	NULL	NULL	gw70_development_131_14_3263_s_235	15201219	(B) GLD-1 binds the GRE and  may repress  pal-1 translation after ribosome loading.	bind
9613	2	3899	5	11	NULL	NULL	NULL	GLD-1	GP		repress		may			pal-1	GP	translation of			NULL		NULL	NULL	NULL	NULL	gw70_development_131_14_3263_s_235	15201219	(B) GLD-1 binds the GRE and  may repress  pal-1 translation after ribosome loading.	bind
9614	3	3899	5	11	NULL	NULL	NULL	statement 2	Process		occurs after					ribosome loading	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_131_14_3263_s_235	15201219	(B) GLD-1 binds the GRE and  may repress  pal-1 translation after ribosome loading.	bind
9455	1	3899	6	11	NULL	NULL	NULL	GLD-1	GP		bind									GRE	NULL		NULL	NULL	NULL	NULL	gw70_development_131_14_3263_s_235	15201219	(B) GLD-1 binds the GRE and  may repress  pal-1 translation after ribosome loading.	bind
9456	2	3899	6	11	NULL	NULL	NULL	GLD-1	GP		repress		may			pal-1	GP	translation of			NULL		NULL	NULL	NULL	NULL	gw70_development_131_14_3263_s_235	15201219	(B) GLD-1 binds the GRE and  may repress  pal-1 translation after ribosome loading.	bind
9457	3	3899	6	11	NULL	NULL	NULL	statement 2	Process		occurs after					ribosome loading	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_131_14_3263_s_235	15201219	(B) GLD-1 binds the GRE and  may repress  pal-1 translation after ribosome loading.	bind
9615	1	3900	5	11	NULL	NULL	NULL	GMAP-210	GP		bind					microtubules	CellComponent	taxol-polymerized			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_1_83_s_270	10189370	(B) GMAP-210  binds to taxol-polymerized microtubules.	bind
9458	1	3900	6	11	NULL	NULL	NULL	GMAP-210	GP		bind					microtubules	CellComponent	taxol-polymerized			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_1_83_s_270	10189370	(B) GMAP-210  binds to taxol-polymerized microtubules.	bind
9616	1	3901	5	11	NULL	NULL	NULL	Bim	GP		bind					Bcl-w	GP				NULL	in epileptic brain	NULL	NULL	NULL	NULL	gw70_jclininvest_113_7_1059_s_268	15057313	(B) Graph showing quantification of higher Bim binding to Bcl-w (OD  units) in epileptic brain.	bind
9459	1	3901	6	11	NULL	NULL	NULL	Bim	GP		bind					Bcl-w	GP				NULL	epileptic brain	NULL	NULL	NULL	NULL	gw70_jclininvest_113_7_1059_s_268	15057313	(B) Graph showing quantification of higher Bim binding to Bcl-w (OD  units) in epileptic brain.	bind
10556	1	3902	5	11	NULL	NULL	NULL	U1A	GP	mutant	bind					PIE RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_9_3163_s_128	12697817	(B) Graphic summary  of the EMSAs in which the  y axis shows the PIE RNA binding activities of the mutant proteins in forming the (U1A)2-PIE RNA complex relative to that of U1Awt, which was set to 1.0.	bind
10557	2	3902	5	11	NULL	NULL	NULL	statement 1	Process		forms					(U1A)2-PIE RNA complex	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_9_3163_s_128	12697817	(B) Graphic summary  of the EMSAs in which the  y axis shows the PIE RNA binding activities of the mutant proteins in forming the (U1A)2-PIE RNA complex relative to that of U1Awt, which was set to 1.0.	bind
9662	1	3902	6	11	NULL	NULL	NULL	U1A	GP	mutant	bind					PIE RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_9_3163_s_128	12697817	(B) Graphic summary  of the EMSAs in which the  y axis shows the PIE RNA binding activities of the mutant proteins in forming the (U1A)2-PIE RNA complex relative to that of U1Awt, which was set to 1.0.	bind
9663	2	3902	6	11	NULL	NULL	NULL	statement 1	Process		forms 					(U1A)2-PIE RNA complex	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_9_3163_s_128	12697817	(B) Graphic summary  of the EMSAs in which the  y axis shows the PIE RNA binding activities of the mutant proteins in forming the (U1A)2-PIE RNA complex relative to that of U1Awt, which was set to 1.0.	bind
9617	1	3904	5	11	NULL	NULL	NULL	GrnCDE			bind					GST-cyclin T1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_5_1688_s_39	12588988	(B) GrnCDE and GEP binding to GST-cyclin T1.	bind
9618	2	3904	5	NULL	NULL	0	NULL	GEP	NULL		bind	NULL				GST-cyclin T1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_5_1688_s_39	12588988	(B) GrnCDE and GEP binding to GST-cyclin T1.	bind
9460	1	3904	6	NULL	NULL	0	NULL	GrnCDE	NULL		bind	NULL				GST-cyclin T1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_5_1688_s_39	12588988	(B) GrnCDE and GEP binding to GST-cyclin T1.	bind
9461	2	3904	6	NULL	NULL	0	NULL	GEP	NULL		bind	NULL				GST-cyclin T1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_5_1688_s_39	12588988	(B) GrnCDE and GEP binding to GST-cyclin T1.	bind
9619	1	3907	5	11	NULL	NULL	NULL	cypin	GP		bind					PSD-95	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_24_3_659_s_97	10595517	(B) GST fusion protein affinity chromatography shows that cypin binding to PSD-95 requires PDZ1 and PDZ2.	bind
9620	2	3907	5	11	NULL	NULL	NULL	statement 1	Process		require								PDZ1		NULL		NULL	NULL	NULL	NULL	gw60_neuron_24_3_659_s_97	10595517	(B) GST fusion protein affinity chromatography shows that cypin binding to PSD-95 requires PDZ1 and PDZ2.	bind
9621	3	3907	5	11	NULL	NULL	NULL	statement 1	Process		require								PDZ2		NULL		NULL	NULL	NULL	NULL	gw60_neuron_24_3_659_s_97	10595517	(B) GST fusion protein affinity chromatography shows that cypin binding to PSD-95 requires PDZ1 and PDZ2.	bind
9462	1	3907	6	11	NULL	NULL	NULL	cypin	GP		bind					PSD-95	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_24_3_659_s_97	10595517	(B) GST fusion protein affinity chromatography shows that cypin binding to PSD-95 requires PDZ1 and PDZ2.	bind
9463	2	3907	6	11	NULL	NULL	NULL	statement 1	Process		requires								PDZ1		NULL		NULL	NULL	NULL	NULL	gw60_neuron_24_3_659_s_97	10595517	(B) GST fusion protein affinity chromatography shows that cypin binding to PSD-95 requires PDZ1 and PDZ2.	bind
9464	3	3907	6	11	NULL	NULL	NULL	statement 1	Process		requires								PDZ2		NULL		NULL	NULL	NULL	NULL	gw60_neuron_24_3_659_s_97	10595517	(B) GST fusion protein affinity chromatography shows that cypin binding to PSD-95 requires PDZ1 and PDZ2.	bind
9622	1	3908	5	11	NULL	NULL	NULL	E1B 19K	GP	deletion mutant	bind					Bax	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_10_6052_s_267	9742122	(B) GST fusion protein binding assay of deletion mutants of E1B 19K binding to Bax and CED-4.	bind
9623	2	3908	5	11	NULL	NULL	NULL	E1B 19K	GP	deletion mutant	bind					CED-4	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_10_6052_s_267	9742122	(B) GST fusion protein binding assay of deletion mutants of E1B 19K binding to Bax and CED-4.	bind
9465	1	3908	6	11	NULL	NULL	NULL	E1B 19K	GP	deletion mutant	bind					Bax	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_10_6052_s_267	9742122	(B) GST fusion protein binding assay of deletion mutants of E1B 19K binding to Bax and CED-4.	bind
9466	2	3908	6	11	NULL	NULL	NULL	E1B 19K	GP	deletion mutant	bind					CED-4	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_10_6052_s_267	9742122	(B) GST fusion protein binding assay of deletion mutants of E1B 19K binding to Bax and CED-4.	bind
9624	1	3909	5	11	NULL	NULL	NULL	yMBF1 protein	GP		bind			D112A		GCN4	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_4971_s_169	9710580	(B) GST pull-down assays for binding of the yMBF1 D112A protein and yMBF1deltaNT to GCN4.	bind
9628	2	3909	5	11	NULL	NULL	NULL	yMBF1	GP		bind			deltaNT		GCN4	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_4971_s_169	9710580	(B) GST pull-down assays for binding of the yMBF1 D112A protein and yMBF1deltaNT to GCN4.	bind
9467	1	3909	6	11	NULL	NULL	NULL	yMBF1	GP		bind			D112A		GCN4	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_4971_s_169	9710580	(B) GST pull-down assays for binding of the yMBF1 D112A protein and yMBF1deltaNT to GCN4.	bind
9468	2	3909	6	11	NULL	NULL	NULL	yMBF1	GP		bind			deltaNT		GCN4	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_4971_s_169	9710580	(B) GST pull-down assays for binding of the yMBF1 D112A protein and yMBF1deltaNT to GCN4.	bind
9629	1	3911	5	11	NULL	NULL	NULL	GST-12S E1A protein	GP		bind					p300	GP		carboxy-terminal fragments ending at amino acid 2414		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_75	10330164	(B) GST-12S and -13S E1A proteins bind to p300 carboxy-terminal fragments ending at amino acids 2414, 1906, and 1542.	bind
9630	2	3911	5	11	NULL	NULL	NULL	GST-12S E1A protein	GP		bind					p300	GP		carboxy-terminal fragments ending at amino acid 1906		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_75	10330164	(B) GST-12S and -13S E1A proteins bind to p300 carboxy-terminal fragments ending at amino acids 2414, 1906, and 1542.	bind
9631	3	3911	5	11	NULL	NULL	NULL	GST-12S E1A protein	GP		bind					p300	GP		carboxy-terminal fragments ending at amino acid 1542		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_75	10330164	(B) GST-12S and -13S E1A proteins bind to p300 carboxy-terminal fragments ending at amino acids 2414, 1906, and 1542.	bind
9632	4	3911	5	11	NULL	NULL	NULL	GST-13S E1A protein	GP		bind					p300	GP		carboxy-terminal fragments ending at amino acid 2414		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_75	10330164	(B) GST-12S and -13S E1A proteins bind to p300 carboxy-terminal fragments ending at amino acids 2414, 1906, and 1542.	bind
9633	5	3911	5	11	NULL	NULL	NULL	GST-13S E1A protein	GP		bind					p300	GP		carboxy-terminal fragments ending at amino acid 1906		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_75	10330164	(B) GST-12S and -13S E1A proteins bind to p300 carboxy-terminal fragments ending at amino acids 2414, 1906, and 1542.	bind
9634	6	3911	5	11	NULL	NULL	NULL	GST-13S E1A protein	GP		bind					p300	GP		carboxy-terminal fragments ending at amino acid 1542		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_75	10330164	(B) GST-12S and -13S E1A proteins bind to p300 carboxy-terminal fragments ending at amino acids 2414, 1906, and 1542.	bind
9469	1	3911	6	11	NULL	NULL	NULL	GST-12S E1A protein	GP		bind					p300	GP		carboxy terminal fragments ending at amino acid 2414		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_75	10330164	(B) GST-12S and -13S E1A proteins bind to p300 carboxy-terminal fragments ending at amino acids 2414, 1906, and 1542.	bind
9470	2	3911	6	11	NULL	NULL	NULL	GST-12S E1A protein	GP		bind					p300	GP		carboxy terminal fragments ending at amino acid 1906		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_75	10330164	(B) GST-12S and -13S E1A proteins bind to p300 carboxy-terminal fragments ending at amino acids 2414, 1906, and 1542.	bind
12304	3	3911	6	11	NULL	NULL	NULL	GST-12S E1A protein	GP		bind					p300	GP		carboxy-terminal fragments ending at amino acid 1542		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_75	10330164	(B) GST-12S and -13S E1A proteins bind to p300 carboxy-terminal fragments ending at amino acids 2414, 1906, and 1542.	bind
12305	4	3911	6	11	NULL	NULL	NULL	GST-13S E1A protein	GP		bind					p300	GP		carboxy terminal fragments ending at amino acid 2414		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_75	10330164	(B) GST-12S and -13S E1A proteins bind to p300 carboxy-terminal fragments ending at amino acids 2414, 1906, and 1542.	bind
12306	5	3911	6	11	NULL	NULL	NULL	GST-13S E1A protein	GP		bind					p300	GP		carboxy terminal fragments ending at amino acid 1906		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_75	10330164	(B) GST-12S and -13S E1A proteins bind to p300 carboxy-terminal fragments ending at amino acids 2414, 1906, and 1542.	bind
12307	6	3911	6	11	NULL	NULL	NULL	GST-13S E1A protein	GP		bind					p300	GP		carboxy terminal fragments ending at amino acid 1542		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_75	10330164	(B) GST-12S and -13S E1A proteins bind to p300 carboxy-terminal fragments ending at amino acids 2414, 1906, and 1542.	bind
9635	1	3918	5	11	NULL	NULL	NULL	HA-Sec4-N133Ip	GP		bind					myc-Ssop	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molbiolcell_10_12_4149_s_248	10588649	(B) HA-Sec4-N133Ip binds myc-Ssop in vitro.	bind
9471	1	3918	6	11	NULL	NULL	NULL	HA-Sec4-N133Ip	GP		bind					myc-Ssop	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molbiolcell_10_12_4149_s_248	10588649	(B) HA-Sec4-N133Ip binds myc-Ssop in vitro.	bind
9636	1	3919	5	11	NULL	NULL	NULL	NF-kappaB	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_104_3_731_s_111	11440805	(b) HDB/SI/MCPO shows a significant increase (+242.6%, paired  t-test;  t=-3.03, DF=4,  P<0.03) in NF- B DNA binding activity following adenosine treatment when compared to ACSF treated samples.	bind
9637	2	3919	5	11	NULL	NULL	NULL	adenosine	NucleicAcid	treatment with	increase		significantly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_104_3_731_s_111	11440805	(b) HDB/SI/MCPO shows a significant increase (+242.6%, paired  t-test;  t=-3.03, DF=4,  P<0.03) in NF- B DNA binding activity following adenosine treatment when compared to ACSF treated samples.	bind
9472	1	3919	6	11	NULL	NULL	NULL	NF-kappaB	GP		bind					DNA 	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_104_3_731_s_111	11440805	(b) HDB/SI/MCPO shows a significant increase (+242.6%, paired  t-test;  t=-3.03, DF=4,  P<0.03) in NF- B DNA binding activity following adenosine treatment when compared to ACSF treated samples.	bind
9473	2	3919	6	11	NULL	NULL	NULL	adenosine 	NucleicAcid	treatment with	increase		significantly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_104_3_731_s_111	11440805	(b) HDB/SI/MCPO shows a significant increase (+242.6%, paired  t-test;  t=-3.03, DF=4,  P<0.03) in NF- B DNA binding activity following adenosine treatment when compared to ACSF treated samples.	bind
9639	1	3921	5	11	NULL	NULL	NULL	SHH:AP	GP		bind					EGL	GP				NULL	P6 cerebellum	NULL	NULL	NULL	NULL	gw60_development_129_9_2223_s_209	11959830	(B) Heparinase I and III treatment results in significantly decreased binding of SHH:AP to the EGL and IGL in sections of P6 cerebellum.	bind
9640	2	3921	5	11	NULL	NULL	NULL	SHH:AP	GP		bind					IGL	GP				NULL	P6 cerebellum	NULL	NULL	NULL	NULL	gw60_development_129_9_2223_s_209	11959830	(B) Heparinase I and III treatment results in significantly decreased binding of SHH:AP to the EGL and IGL in sections of P6 cerebellum.	bind
9641	3	3921	5	11	NULL	NULL	NULL	Heparinase I	GP	treatment	decrease		significantly			statement 1	Process				NULL	P6 cerebellum	NULL	NULL	NULL	NULL	gw60_development_129_9_2223_s_209	11959830	(B) Heparinase I and III treatment results in significantly decreased binding of SHH:AP to the EGL and IGL in sections of P6 cerebellum.	bind
9642	4	3921	5	11	NULL	NULL	NULL	Heparinase I	GP	treatment	decrease		significantly			statement 2	Process				NULL	P6 cerebellum	NULL	NULL	NULL	NULL	gw60_development_129_9_2223_s_209	11959830	(B) Heparinase I and III treatment results in significantly decreased binding of SHH:AP to the EGL and IGL in sections of P6 cerebellum.	bind
9643	5	3921	5	11	NULL	NULL	NULL	Heparinase III	GP	treatment	decrease		significantly			statement 1	Process				NULL	P6 cerebellum	NULL	NULL	NULL	NULL	gw60_development_129_9_2223_s_209	11959830	(B) Heparinase I and III treatment results in significantly decreased binding of SHH:AP to the EGL and IGL in sections of P6 cerebellum.	bind
9644	6	3921	5	11	NULL	NULL	NULL	Heparinase III	GP	treatment	decrease		significantly			statement 2	Process				NULL	P6 cerebellum	NULL	NULL	NULL	NULL	gw60_development_129_9_2223_s_209	11959830	(B) Heparinase I and III treatment results in significantly decreased binding of SHH:AP to the EGL and IGL in sections of P6 cerebellum.	bind
9474	1	3921	6	11	NULL	NULL	NULL	SHH:AP	GP		bind					EGL	GP				NULL	sections of P6 cerebellum	NULL	NULL	NULL	NULL	gw60_development_129_9_2223_s_209	11959830	(B) Heparinase I and III treatment results in significantly decreased binding of SHH:AP to the EGL and IGL in sections of P6 cerebellum.	bind
9475	2	3921	6	NULL	NULL	0	NULL	SHH:AP	NULL		bind	NULL				IGL	NULL				NULL	sections of P6 cerebellum	0	NULL	NULL	NULL	gw60_development_129_9_2223_s_209	11959830	(B) Heparinase I and III treatment results in significantly decreased binding of SHH:AP to the EGL and IGL in sections of P6 cerebellum.	bind
9476	3	3921	6	NULL	NULL	0	NULL	Heparinase I	NULL		decreases	NULL	significantly			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_development_129_9_2223_s_209	11959830	(B) Heparinase I and III treatment results in significantly decreased binding of SHH:AP to the EGL and IGL in sections of P6 cerebellum.	bind
9477	4	3921	6	NULL	NULL	0	NULL	Heparinase III	NULL		decreases	NULL	significantly			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_development_129_9_2223_s_209	11959830	(B) Heparinase I and III treatment results in significantly decreased binding of SHH:AP to the EGL and IGL in sections of P6 cerebellum.	bind
12308	5	3921	6	11	NULL	NULL	NULL	Heparinase I	GP		decreases		significantly			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_development_129_9_2223_s_209	11959830	(B) Heparinase I and III treatment results in significantly decreased binding of SHH:AP to the EGL and IGL in sections of P6 cerebellum.	bind
12309	6	3921	6	NULL	NULL	0	NULL	Heparinase III	NULL		decreases	NULL	significantly			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_development_129_9_2223_s_209	11959830	(B) Heparinase I and III treatment results in significantly decreased binding of SHH:AP to the EGL and IGL in sections of P6 cerebellum.	bind
9645	1	3922	5	11	NULL	NULL	NULL	BTAF1	GP		bind					TBP	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_22_10072_s_112	15509807	(B) Hexokinase activity is  necessary to abolish NC2alpha-mediated binding of BTAF1 and TBP. RK13 cell lysate (1 mul) containing overexpressed  BTAF1 was incubated with glutathione-agarose beads coated with GST-TBP (lanes 3 to  6 and 8 to 11) or GST-deltaTFIIS (lanes 7 and 12) in the absence (lanes 3, 7, 8, and 12) or presence of 6.5 pmol  of hisNC2alpha (lanes 4 and 9), hisNC2beta (lanes 5 and 10), and NC2(alpha/hisbeta) (lanes 6 and 11).	bind
9646	2	3922	5	11	NULL	NULL	NULL	NC2alpha	GP		mediate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_22_10072_s_112	15509807	(B) Hexokinase activity is  necessary to abolish NC2alpha-mediated binding of BTAF1 and TBP. RK13 cell lysate (1 mul) containing overexpressed  BTAF1 was incubated with glutathione-agarose beads coated with GST-TBP (lanes 3 to  6 and 8 to 11) or GST-deltaTFIIS (lanes 7 and 12) in the absence (lanes 3, 7, 8, and 12) or presence of 6.5 pmol  of hisNC2alpha (lanes 4 and 9), hisNC2beta (lanes 5 and 10), and NC2(alpha/hisbeta) (lanes 6 and 11).	bind
9647	3	3922	5	11	NULL	NULL	NULL	hexokinase 	GP	activity of	abolish					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_22_10072_s_112	15509807	(B) Hexokinase activity is  necessary to abolish NC2alpha-mediated binding of BTAF1 and TBP. RK13 cell lysate (1 mul) containing overexpressed  BTAF1 was incubated with glutathione-agarose beads coated with GST-TBP (lanes 3 to  6 and 8 to 11) or GST-deltaTFIIS (lanes 7 and 12) in the absence (lanes 3, 7, 8, and 12) or presence of 6.5 pmol  of hisNC2alpha (lanes 4 and 9), hisNC2beta (lanes 5 and 10), and NC2(alpha/hisbeta) (lanes 6 and 11).	bind
9664	1	3922	6	11	NULL	NULL	NULL	BTAF1	GP		bind					TBP	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_22_10072_s_112	15509807	(B) Hexokinase activity is  necessary to abolish NC2alpha-mediated binding of BTAF1 and TBP. RK13 cell lysate (1 mul) containing overexpressed  BTAF1 was incubated with glutathione-agarose beads coated with GST-TBP (lanes 3 to  6 and 8 to 11) or GST-deltaTFIIS (lanes 7 and 12) in the absence (lanes 3, 7, 8, and 12) or presence of 6.5 pmol  of hisNC2alpha (lanes 4 and 9), hisNC2beta (lanes 5 and 10), and NC2(alpha/hisbeta) (lanes 6 and 11).	bind
9665	2	3922	6	11	NULL	NULL	NULL	NC2alpha	GP		mediates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_22_10072_s_112	15509807	(B) Hexokinase activity is  necessary to abolish NC2alpha-mediated binding of BTAF1 and TBP. RK13 cell lysate (1 mul) containing overexpressed  BTAF1 was incubated with glutathione-agarose beads coated with GST-TBP (lanes 3 to  6 and 8 to 11) or GST-deltaTFIIS (lanes 7 and 12) in the absence (lanes 3, 7, 8, and 12) or presence of 6.5 pmol  of hisNC2alpha (lanes 4 and 9), hisNC2beta (lanes 5 and 10), and NC2(alpha/hisbeta) (lanes 6 and 11).	bind
9666	3	3922	6	11	NULL	NULL	NULL	hexokinase	GP	activity of	abolish					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_22_10072_s_112	15509807	(B) Hexokinase activity is  necessary to abolish NC2alpha-mediated binding of BTAF1 and TBP. RK13 cell lysate (1 mul) containing overexpressed  BTAF1 was incubated with glutathione-agarose beads coated with GST-TBP (lanes 3 to  6 and 8 to 11) or GST-deltaTFIIS (lanes 7 and 12) in the absence (lanes 3, 7, 8, and 12) or presence of 6.5 pmol  of hisNC2alpha (lanes 4 and 9), hisNC2beta (lanes 5 and 10), and NC2(alpha/hisbeta) (lanes 6 and 11).	bind
9648	1	3923	5	11	NULL	NULL	NULL	Hif-1	GP		bind									HRE	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3163_s_219	15798202	(B) Hif-1 and Hif-2 HRE binding activity by EMSA.	bind
9649	2	3923	5	11	NULL	NULL	NULL	Hif-2	GP		bind									HRE	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3163_s_219	15798202	(B) Hif-1 and Hif-2 HRE binding activity by EMSA.	bind
9478	1	3923	6	11	NULL	NULL	NULL	HIF-1	GP		bind									HRE	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3163_s_219	15798202	(B) Hif-1 and Hif-2 HRE binding activity by EMSA.	bind
9479	2	3923	6	11	NULL	NULL	NULL	HIF-2	GP		bind									HRE	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3163_s_219	15798202	(B) Hif-1 and Hif-2 HRE binding activity by EMSA.	bind
9650	1	3924	5	11	NULL	NULL	NULL	Hir1p	GP		bind					Asf1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_7_463_s_193	11412995	(b) Hir1p and Hir2p coimmunoprecipitate with Asf1p.	bind
9651	2	3924	5	11	NULL	NULL	NULL	Hir2p	GP		bind					Asf1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_7_463_s_193	11412995	(b) Hir1p and Hir2p coimmunoprecipitate with Asf1p.	bind
9480	1	3924	6	11	NULL	NULL	NULL	Hir1p	GP		bind					Asf1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_7_463_s_193	11412995	(b) Hir1p and Hir2p coimmunoprecipitate with Asf1p.	bind
9481	2	3924	6	11	NULL	NULL	NULL	Hir2p	GP		bind					Asf1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_7_463_s_193	11412995	(b) Hir1p and Hir2p coimmunoprecipitate with Asf1p.	bind
9652	1	3926	5	11	NULL	NULL	NULL	Arr2	GP		bind					membranes	CellComponent	rhodopsin-containing			NULL		NULL	NULL	NULL	NULL	gw60_neuron_28_1_129_s_159	11086989	(B) Histogram quantifying the percent of Arr2 bound to rhodopsin-containing membranes after treatment with blue light (B) or blue light followed by orange light (BO).	bind
9482	1	3926	6	11	NULL	NULL	NULL	Arr2	GP		bind					membranes	CellComponent	rhodopsin-containing			NULL		NULL	NULL	NULL	NULL	gw60_neuron_28_1_129_s_159	11086989	(B) Histogram quantifying the percent of Arr2 bound to rhodopsin-containing membranes after treatment with blue light (B) or blue light followed by orange light (BO).	bind
9653	1	3927	5	11	NULL	NULL	NULL	hMSH2-hMSH6	GP		bind					DNA mismatched 	NucleicAcid	nicked;; circular 		O-G/T	NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_2_255_s_100	10078208	(B) hMSH2-hMSH6 (65 nM) binding a nicked circular 2.9 kb mismatched (O-G/T) or homoduplex (O-G/C) DNA.	bind
9654	2	3927	5	11	NULL	NULL	NULL	hMSH2-hMSH6	GP		bind					DNA homoduplex	NucleicAcid	nicked;; circular		O-G/C	NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_2_255_s_100	10078208	(B) hMSH2-hMSH6 (65 nM) binding a nicked circular 2.9 kb mismatched (O-G/T) or homoduplex (O-G/C) DNA.	bind
9536	1	3927	6	11	NULL	NULL	NULL	 hMSH2-hMSH6	GP		bind					mismatched DNA	NucleicAcid	nicked;; circular 		O-G/T	NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_2_255_s_100	10078208	(B) hMSH2-hMSH6 (65 nM) binding a nicked circular 2.9 kb mismatched (O-G/T) or homoduplex (O-G/C) DNA.	bind
9537	2	3927	6	11	NULL	NULL	NULL	hMSH2-hMSH6	GP		bind					homoduplex DNA	NucleicAcid	nicked;; circular		O-G/C	NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_2_255_s_100	10078208	(B) hMSH2-hMSH6 (65 nM) binding a nicked circular 2.9 kb mismatched (O-G/T) or homoduplex (O-G/C) DNA.	bind
9655	1	3929	5	11	NULL	NULL	NULL	HrpR	GP		bind					protein	GP	E. coli			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_19_5589_s_245	11544221	(B) HrpR binding to an  E. coli protein-loaded column.	bind
9538	1	3929	6	11	NULL	NULL	NULL	HrpR	GP		bind					protein	GP	E.coli			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_19_5589_s_245	11544221	(B) HrpR binding to an  E. coli protein-loaded column.	bind
9656	1	3930	5	11	NULL	NULL	NULL	Hsp104	GP		bind					Sti1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_22_7569_s_134	11604493	(B) Hsp104 and Hsp90 binding to Sti1 requires TPR1 and TPR2, respectively.	bind
9657	2	3930	5	11	NULL	NULL	NULL	statement 1	Process		require					TPR1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_22_7569_s_134	11604493	(B) Hsp104 and Hsp90 binding to Sti1 requires TPR1 and TPR2, respectively.	bind
9658	3	3930	5	11	NULL	NULL	NULL	Hsp90	GP		bind					Sti1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_22_7569_s_134	11604493	(B) Hsp104 and Hsp90 binding to Sti1 requires TPR1 and TPR2, respectively.	bind
9691	4	3930	5	11	NULL	NULL	NULL	statement 3	Process		require					TPR2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_22_7569_s_134	11604493	(B) Hsp104 and Hsp90 binding to Sti1 requires TPR1 and TPR2, respectively.	bind
9539	1	3930	6	11	NULL	NULL	NULL	Hsp104	GP		bind					Sti1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_22_7569_s_134	11604493	(B) Hsp104 and Hsp90 binding to Sti1 requires TPR1 and TPR2, respectively.	bind
9540	2	3930	6	11	NULL	NULL	NULL	Hsp90	GP		bind					Sti1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_22_7569_s_134	11604493	(B) Hsp104 and Hsp90 binding to Sti1 requires TPR1 and TPR2, respectively.	bind
9541	3	3930	6	11	NULL	NULL	NULL	statement 1	Process		requires					TPR1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_22_7569_s_134	11604493	(B) Hsp104 and Hsp90 binding to Sti1 requires TPR1 and TPR2, respectively.	bind
9544	4	3930	6	11	NULL	NULL	NULL	statement 2	Process		requires					TPR2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_22_7569_s_134	11604493	(B) Hsp104 and Hsp90 binding to Sti1 requires TPR1 and TPR2, respectively.	bind
9701	1	3931	5	11	NULL	NULL	NULL	mediator		human	bind					DNA	NucleicAcid			promoter	NULL		NULL	NULL	NULL	NULL	gw60_currbiol_13_9_772_s_19	12725737	(B) Human mediator and DA bind cooperatively to promoter DNA.	bind
9702	2	3931	5	11	NULL	NULL	NULL	DA	GP	human	bind					DNA	NucleicAcid			promoter	NULL		NULL	NULL	NULL	NULL	gw60_currbiol_13_9_772_s_19	12725737	(B) Human mediator and DA bind cooperatively to promoter DNA.	bind
9703	3	3931	5	11	NULL	NULL	NULL	statement 1	Process		occurs in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_13_9_772_s_19	12725737	(B) Human mediator and DA bind cooperatively to promoter DNA.	bind
9545	1	3931	6	11	NULL	NULL	NULL	mediator		human	bind					DNA	NucleicAcid			promoter	NULL		NULL	NULL	NULL	NULL	gw60_currbiol_13_9_772_s_19	12725737	(B) Human mediator and DA bind cooperatively to promoter DNA.	bind
9546	2	3931	6	11	NULL	NULL	NULL	DA	GP		bind					DNA	NucleicAcid			promoter	NULL		NULL	NULL	NULL	NULL	gw60_currbiol_13_9_772_s_19	12725737	(B) Human mediator and DA bind cooperatively to promoter DNA.	bind
9547	3	3931	6	11	NULL	NULL	NULL	statement 1	Process		occurs in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_13_9_772_s_19	12725737	(B) Human mediator and DA bind cooperatively to promoter DNA.	bind
9704	1	3932	5	11	NULL	NULL	NULL	p70 MGR	GP	human	bind					En-1	GP	human		promoter	NULL		NULL	NULL	NULL	NULL	gw60_mechdev_114_1_37_s_177	12175488	(B) Human p70 MGR binds to the human En-1 promoter.	bind
9548	1	3932	6	11	NULL	NULL	NULL	p70 MGR	GP	human	bind					En-1	GP	human		promoter	NULL		NULL	NULL	NULL	NULL	gw60_mechdev_114_1_37_s_177	12175488	(B) Human p70 MGR binds to the human En-1 promoter.	bind
9705	1	3933	5	11	NULL	NULL	NULL	hRNF5	GP		bind					paxillin	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_15_5331_s_131	12861019	(B) Human RNF5  (hRNF5) binds to paxillin.	bind
9706	2	3933	5	11	NULL	NULL	NULL	hRNF5	GP		is					human RNF5	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_15_5331_s_131	12861019	(B) Human RNF5  (hRNF5) binds to paxillin.	bind
9549	1	3933	6	11	NULL	NULL	NULL	hRNF5	GP		bind					paxillin	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_15_5331_s_131	12861019	(B) Human RNF5  (hRNF5) binds to paxillin.	bind
9550	2	3933	6	11	NULL	NULL	NULL	hRNF5	GP		is					human RNF5	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_15_5331_s_131	12861019	(B) Human RNF5  (hRNF5) binds to paxillin.	bind
9707	1	3935	5	11	NULL	NULL	NULL	HVEM:Fc	Organism		bind					T cells	Cell	activated;; human;; peripheral blood			NULL		NULL	NULL	NULL	NULL	gw60_immunity_8_1_21_s_52	9462508	(B) HVEM:Fc binds activated T cells from human peripheral blood.	bind
9551	1	3935	6	11	NULL	NULL	NULL	HVEM:Fc	Organism		bind					T cells 	Cell	activated;; human;; peripheral blood			NULL		NULL	NULL	NULL	NULL	gw60_immunity_8_1_21_s_52	9462508	(B) HVEM:Fc binds activated T cells from human peripheral blood.	bind
9708	1	3936	5	11	NULL	NULL	NULL	E47 homodimers	GP		bind		sequence specific			MEF-1 oligodeoxynucleotide	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_313	11940648	(B) Id2 inhibits the sequence-specific binding of E47 homodimers and MyoD-E47 heterodimers to the MEF-1 oligodeoxynucleotide in vitro, and p204 overcomes the inhibition.	bind
9709	2	3936	5	11	NULL	NULL	NULL	MyoD-E47 heterodimers	GP		bind		sequence specific			MEF-1 oligodeoxynucleotide	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_313	11940648	(B) Id2 inhibits the sequence-specific binding of E47 homodimers and MyoD-E47 heterodimers to the MEF-1 oligodeoxynucleotide in vitro, and p204 overcomes the inhibition.	bind
9710	3	3936	5	11	NULL	NULL	NULL	Id2	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_313	11940648	(B) Id2 inhibits the sequence-specific binding of E47 homodimers and MyoD-E47 heterodimers to the MEF-1 oligodeoxynucleotide in vitro, and p204 overcomes the inhibition.	bind
9711	4	3936	5	11	NULL	NULL	NULL	Id2	GP		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_313	11940648	(B) Id2 inhibits the sequence-specific binding of E47 homodimers and MyoD-E47 heterodimers to the MEF-1 oligodeoxynucleotide in vitro, and p204 overcomes the inhibition.	bind
9712	5	3936	5	11	NULL	NULL	NULL	p204	GP		overcomes					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_313	11940648	(B) Id2 inhibits the sequence-specific binding of E47 homodimers and MyoD-E47 heterodimers to the MEF-1 oligodeoxynucleotide in vitro, and p204 overcomes the inhibition.	bind
9713	6	3936	5	11	NULL	NULL	NULL	p204	GP		overcomes					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_313	11940648	(B) Id2 inhibits the sequence-specific binding of E47 homodimers and MyoD-E47 heterodimers to the MEF-1 oligodeoxynucleotide in vitro, and p204 overcomes the inhibition.	bind
9557	1	3936	6	11	NULL	NULL	NULL	E47 homodimers	GP		bind					MEF-1 oligodeoxynucleotide	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_313	11940648	(B) Id2 inhibits the sequence-specific binding of E47 homodimers and MyoD-E47 heterodimers to the MEF-1 oligodeoxynucleotide in vitro, and p204 overcomes the inhibition.	bind
9558	2	3936	6	11	NULL	NULL	NULL	MyoD-E47 heterodimers	GP		bind					MEF-1 oligodeoxynucleotide	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_313	11940648	(B) Id2 inhibits the sequence-specific binding of E47 homodimers and MyoD-E47 heterodimers to the MEF-1 oligodeoxynucleotide in vitro, and p204 overcomes the inhibition.	bind
9559	3	3936	6	NULL	NULL	0	NULL	Id2	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_313	11940648	(B) Id2 inhibits the sequence-specific binding of E47 homodimers and MyoD-E47 heterodimers to the MEF-1 oligodeoxynucleotide in vitro, and p204 overcomes the inhibition.	bind
9560	4	3936	6	NULL	NULL	0	NULL	Id2	NULL		inhibits	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_313	11940648	(B) Id2 inhibits the sequence-specific binding of E47 homodimers and MyoD-E47 heterodimers to the MEF-1 oligodeoxynucleotide in vitro, and p204 overcomes the inhibition.	bind
9561	5	3936	6	NULL	NULL	0	NULL	p204	NULL		overcomes	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_313	11940648	(B) Id2 inhibits the sequence-specific binding of E47 homodimers and MyoD-E47 heterodimers to the MEF-1 oligodeoxynucleotide in vitro, and p204 overcomes the inhibition.	bind
9562	6	3936	6	NULL	NULL	0	NULL	p204	NULL		overcomes	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_313	11940648	(B) Id2 inhibits the sequence-specific binding of E47 homodimers and MyoD-E47 heterodimers to the MEF-1 oligodeoxynucleotide in vitro, and p204 overcomes the inhibition.	bind
9714	1	3940	5	11	NULL	NULL	NULL	IHF	GP		bind					 Ppac	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_7_2215_s_94	15028709	(B) IHF binding to the  Ppac promoter.	bind
9563	1	3940	6	11	NULL	NULL	NULL	IHF	GP		bind					Ppac	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_7_2215_s_94	15028709	(B) IHF binding to the  Ppac promoter.	bind
9715	1	3945	5	11	NULL	NULL	NULL	EMILIN-1	GP		bind					elastin	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_2_638_s_238	14701737	(B) Immunoprecipitation assays  showing binding of EMILIN-1 to elastin and fibulin-5.	bind
9716	2	3945	5	11	NULL	NULL	NULL	EMILIN-1	GP		bind					fibulin-5	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_2_638_s_238	14701737	(B) Immunoprecipitation assays  showing binding of EMILIN-1 to elastin and fibulin-5.	bind
9564	1	3945	6	11	NULL	NULL	NULL	EMILIN-1	GP		bind					elastin	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_2_638_s_238	14701737	(B) Immunoprecipitation assays  showing binding of EMILIN-1 to elastin and fibulin-5.	bind
9565	2	3945	6	11	NULL	NULL	NULL	EMILIN-1	GP		bind					fibulin-5	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_2_638_s_238	14701737	(B) Immunoprecipitation assays  showing binding of EMILIN-1 to elastin and fibulin-5.	bind
9718	2	3946	5	10	NULL	0	NULL	statement 1			in the absence of					antiserum					NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_44_6_817_s_249	12681380	(B) Immunoprecipitations performed in the absence of antiserum demonstrate that  syntaxin 1 binds directly to protein A sepharose.	bind
9566	1	3946	6	NULL	NULL	0	NULL	syntaxin 1	NULL		bind	NULL	directly			Protein A	NULL				NULL		0	NULL	NULL	NULL	gw70_neuropharmacology_44_6_817_s_249	12681380	(B) Immunoprecipitations performed in the absence of antiserum demonstrate that  syntaxin 1 binds directly to protein A sepharose.	bind
53714	2	3946	6	10	NULL	0	NULL	statement 1			in the absence of					antiserum					NULL		0	NULL	NULL	NULL	gw70_neuropharmacology_44_6_817_s_249	12681380	(B) Immunoprecipitations performed in the absence of antiserum demonstrate that  syntaxin 1 binds directly to protein A sepharose.	bind
9717	1	3948	5	11	NULL	NULL	NULL	syntaxin 1	GP		bind		directly			protein A	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_110_3_349_s_173	12176322	(B) Importin-alpha can bind NLS and the N terminus of Npap60 simultaneously.	bind
9719	1	3948	5	11	NULL	NULL	NULL	importin-alpha	GP		bind					Npap60	GP		NLS		NULL		NULL	NULL	NULL	NULL	gw60_cell_110_3_349_s_173	12176322	(B) Importin-alpha can bind NLS and the N terminus of Npap60 simultaneously.	bind
9720	2	3948	5	11	NULL	NULL	NULL	importin-alpha	GP		bind					Npap60	GP		N terminus		NULL		NULL	NULL	NULL	NULL	gw60_cell_110_3_349_s_173	12176322	(B) Importin-alpha can bind NLS and the N terminus of Npap60 simultaneously.	bind
9721	3	3948	5	11	NULL	NULL	NULL	statement 1	Process		occurs simultaneously with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_110_3_349_s_173	12176322	(B) Importin-alpha can bind NLS and the N terminus of Npap60 simultaneously.	bind
9567	1	3948	6	11	NULL	NULL	NULL	Importin-alpha	GP		bind					NLS	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_110_3_349_s_173	12176322	(B) Importin-alpha can bind NLS and the N terminus of Npap60 simultaneously.	bind
9568	2	3948	6	11	NULL	NULL	NULL	Importin alpha	GP		bind					Npap60	GP		N-terminus		NULL		NULL	NULL	NULL	NULL	gw60_cell_110_3_349_s_173	12176322	(B) Importin-alpha can bind NLS and the N terminus of Npap60 simultaneously.	bind
12503	3	3948	6	11	NULL	NULL	NULL	statement 1	Process		occurs simultaneously with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_110_3_349_s_173	12176322	(B) Importin-alpha can bind NLS and the N terminus of Npap60 simultaneously.	bind
9722	1	3949	5	11	NULL	NULL	NULL	cyclin D1	GP		bind					CCND1 gene	GP			upstream regulatory region	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_16_7260_s_258	15282324	(B) In  vitro binding of cyclin D1 and pRb to the upstream regulatory region of the  CCND1 gene.	bind
9723	2	3949	5	11	NULL	NULL	NULL	pRb	GP		bind					CCND1 gene	GP			upstream regulatory region	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_16_7260_s_258	15282324	(B) In  vitro binding of cyclin D1 and pRb to the upstream regulatory region of the  CCND1 gene.	bind
9569	1	3949	6	11	NULL	NULL	NULL	Cyclin D1	GP		bind					CCND1 gene	GP			upstream regulatory region	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_16_7260_s_258	15282324	(B) In  vitro binding of cyclin D1 and pRb to the upstream regulatory region of the  CCND1 gene.	bind
9570	2	3949	6	11	NULL	NULL	NULL	pRb	GP		bind					CCND1 gene	GP			upstream regulatory region	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_16_7260_s_258	15282324	(B) In  vitro binding of cyclin D1 and pRb to the upstream regulatory region of the  CCND1 gene.	bind
9724	1	3950	5	11	NULL	NULL	NULL	FGF-1	GP		bind		high affinity			FGFR2	GP				NULL	cells expressing cell surface proteoglycans	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_6754_s_368	10490614	(B) In cells where cell surface proteoglycans are present, FGF-1 binds to FGFR2 with a high affinity through interaction with the heparan sulfate glycosaminoglycan moiety and transmits moderate downstream signals.	bind
9728	2	3950	5	11	NULL	NULL	NULL	FGF-1	GP		interacts with					heparan sulfate glycosaminoglycan	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_6754_s_368	10490614	(B) In cells where cell surface proteoglycans are present, FGF-1 binds to FGFR2 with a high affinity through interaction with the heparan sulfate glycosaminoglycan moiety and transmits moderate downstream signals.	bind
9729	4	3950	5	11	NULL	NULL	NULL	statement 2	Process		transmits					downstream signals	Process	moderate			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_6754_s_368	10490614	(B) In cells where cell surface proteoglycans are present, FGF-1 binds to FGFR2 with a high affinity through interaction with the heparan sulfate glycosaminoglycan moiety and transmits moderate downstream signals.	bind
13001	3	3950	5	11	NULL	NULL	NULL	statement 1	Process		occurs through					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_6754_s_368	10490614	(B) In cells where cell surface proteoglycans are present, FGF-1 binds to FGFR2 with a high affinity through interaction with the heparan sulfate glycosaminoglycan moiety and transmits moderate downstream signals.	bind
9571	1	3950	6	11	NULL	NULL	NULL	FGF-1	GP		bind		high affinity			FGFR2	GP				NULL	cells expressing cell surface proteoglycans	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_6754_s_368	10490614	(B) In cells where cell surface proteoglycans are present, FGF-1 binds to FGFR2 with a high affinity through interaction with the heparan sulfate glycosaminoglycan moiety and transmits moderate downstream signals.	bind
9667	2	3950	6	11	NULL	NULL	NULL	FGF-1	GP		interacts with					heparan sulfate glycosaminoglycan	Chemical				NULL	cells expressing cell surface proteoglycans	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_6754_s_368	10490614	(B) In cells where cell surface proteoglycans are present, FGF-1 binds to FGFR2 with a high affinity through interaction with the heparan sulfate glycosaminoglycan moiety and transmits moderate downstream signals.	bind
9668	3	3950	6	11	NULL	NULL	NULL	statement 1	Process		occurs through					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_6754_s_368	10490614	(B) In cells where cell surface proteoglycans are present, FGF-1 binds to FGFR2 with a high affinity through interaction with the heparan sulfate glycosaminoglycan moiety and transmits moderate downstream signals.	bind
9669	4	3950	6	11	NULL	NULL	NULL	FGF-1	GP		transmits					downstream signals	Process	moderate			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_6754_s_368	10490614	(B) In cells where cell surface proteoglycans are present, FGF-1 binds to FGFR2 with a high affinity through interaction with the heparan sulfate glycosaminoglycan moiety and transmits moderate downstream signals.	bind
10558	1	3951	5	11	NULL	NULL	NULL	RITS complex	GP		assembles at 									cenH	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2331_s_46	15743828	(B) In contrast, the RNAi-dependent assembly of the RITS complex at  cenH or centromeric sequences promotes recruitment of Clr4 to these sequences and is important  for establishment of silencing.	bind
10559	2	3951	5	11	NULL	NULL	NULL	RITS complex	GP		assembles at									centromeric sequences	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2331_s_46	15743828	(B) In contrast, the RNAi-dependent assembly of the RITS complex at  cenH or centromeric sequences promotes recruitment of Clr4 to these sequences and is important  for establishment of silencing.	bind
10560	5	3951	5	11	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2331_s_46	15743828	(B) In contrast, the RNAi-dependent assembly of the RITS complex at  cenH or centromeric sequences promotes recruitment of Clr4 to these sequences and is important  for establishment of silencing.	bind
10561	3	3951	5	11	NULL	NULL	NULL	statement 1	Process		is dependent on					RNAi	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2331_s_46	15743828	(B) In contrast, the RNAi-dependent assembly of the RITS complex at  cenH or centromeric sequences promotes recruitment of Clr4 to these sequences and is important  for establishment of silencing.	bind
10562	4	3951	5	11	NULL	NULL	NULL	statement 2	Process		is dependent on					RNAi	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2331_s_46	15743828	(B) In contrast, the RNAi-dependent assembly of the RITS complex at  cenH or centromeric sequences promotes recruitment of Clr4 to these sequences and is important  for establishment of silencing.	bind
10563	6	3951	5	11	NULL	NULL	NULL	Clr4	GP		is recruited to									cenH	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2331_s_46	15743828	(B) In contrast, the RNAi-dependent assembly of the RITS complex at  cenH or centromeric sequences promotes recruitment of Clr4 to these sequences and is important  for establishment of silencing.	bind
10564	7	3951	5	11	NULL	NULL	NULL	statement 3	Process		promote					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2331_s_46	15743828	(B) In contrast, the RNAi-dependent assembly of the RITS complex at  cenH or centromeric sequences promotes recruitment of Clr4 to these sequences and is important  for establishment of silencing.	bind
10565	8	3951	5	11	NULL	NULL	NULL	Clr4	GP		is recruited to									centromeric sequences	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2331_s_46	15743828	(B) In contrast, the RNAi-dependent assembly of the RITS complex at  cenH or centromeric sequences promotes recruitment of Clr4 to these sequences and is important  for establishment of silencing.	bind
10566	9	3951	5	11	NULL	NULL	NULL	statement 4	Process		promote					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2331_s_46	15743828	(B) In contrast, the RNAi-dependent assembly of the RITS complex at  cenH or centromeric sequences promotes recruitment of Clr4 to these sequences and is important  for establishment of silencing.	bind
10567	10	3951	5	11	NULL	NULL	NULL	statement 7	Process		important for					silencing	Process	establishment of 			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2331_s_46	15743828	(B) In contrast, the RNAi-dependent assembly of the RITS complex at  cenH or centromeric sequences promotes recruitment of Clr4 to these sequences and is important  for establishment of silencing.	bind
10568	11	3951	5	11	NULL	NULL	NULL	statement 9	Process		important for					silencing	Process	establishment of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2331_s_46	15743828	(B) In contrast, the RNAi-dependent assembly of the RITS complex at  cenH or centromeric sequences promotes recruitment of Clr4 to these sequences and is important  for establishment of silencing.	bind
53776	12	3951	5	11	NULL	NULL	NULL	statement 4	Process		promote					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2331_s_46	15743828	(B) In contrast, the RNAi-dependent assembly of the RITS complex at  cenH or centromeric sequences promotes recruitment of Clr4 to these sequences and is important  for establishment of silencing.	bind
53777	13	3951	5	11	NULL	NULL	NULL	statement 3	Process		promote					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2331_s_46	15743828	(B) In contrast, the RNAi-dependent assembly of the RITS complex at  cenH or centromeric sequences promotes recruitment of Clr4 to these sequences and is important  for establishment of silencing.	bind
53778	14	3951	5	11	NULL	NULL	NULL	statement 12	Process		important for					silencing	Process	establishment of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2331_s_46	15743828	(B) In contrast, the RNAi-dependent assembly of the RITS complex at  cenH or centromeric sequences promotes recruitment of Clr4 to these sequences and is important  for establishment of silencing.	bind
53779	15	3951	5	11	NULL	NULL	NULL	statement 13	Process		important for					silencing	Process	establishment of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2331_s_46	15743828	(B) In contrast, the RNAi-dependent assembly of the RITS complex at  cenH or centromeric sequences promotes recruitment of Clr4 to these sequences and is important  for establishment of silencing.	bind
16271	1	3951	6	11	NULL	NULL	NULL	RITS complex	GP		assembles at									cenH sequences	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2331_s_46	15743828	(B) In contrast, the RNAi-dependent assembly of the RITS complex at  cenH or centromeric sequences promotes recruitment of Clr4 to these sequences and is important  for establishment of silencing.	bind
16272	2	3951	6	11	NULL	NULL	NULL	RITS complex	GP		assembles at									centromeric sequences	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2331_s_46	15743828	(B) In contrast, the RNAi-dependent assembly of the RITS complex at  cenH or centromeric sequences promotes recruitment of Clr4 to these sequences and is important  for establishment of silencing.	bind
16273	3	3951	6	11	NULL	NULL	NULL	statement 1	Process		is dependent on					RNAi	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2331_s_46	15743828	(B) In contrast, the RNAi-dependent assembly of the RITS complex at  cenH or centromeric sequences promotes recruitment of Clr4 to these sequences and is important  for establishment of silencing.	bind
16274	4	3951	6	11	NULL	NULL	NULL	statement 2	Process		is dependent on					RNAi	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2331_s_46	15743828	(B) In contrast, the RNAi-dependent assembly of the RITS complex at  cenH or centromeric sequences promotes recruitment of Clr4 to these sequences and is important  for establishment of silencing.	bind
16275	5	3951	6	11	NULL	NULL	NULL	Clr4	GP		is recruited on									cenH sequences	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2331_s_46	15743828	(B) In contrast, the RNAi-dependent assembly of the RITS complex at  cenH or centromeric sequences promotes recruitment of Clr4 to these sequences and is important  for establishment of silencing.	bind
16277	6	3951	6	11	NULL	NULL	NULL	Clr4	GP		is recruited on									centromeric sequences	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2331_s_46	15743828	(B) In contrast, the RNAi-dependent assembly of the RITS complex at  cenH or centromeric sequences promotes recruitment of Clr4 to these sequences and is important  for establishment of silencing.	bind
16278	7	3951	6	11	NULL	NULL	NULL	statement 1	Process		promotes					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2331_s_46	15743828	(B) In contrast, the RNAi-dependent assembly of the RITS complex at  cenH or centromeric sequences promotes recruitment of Clr4 to these sequences and is important  for establishment of silencing.	bind
16279	8	3951	6	11	NULL	NULL	NULL	statement 1	Process		promotes					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2331_s_46	15743828	(B) In contrast, the RNAi-dependent assembly of the RITS complex at  cenH or centromeric sequences promotes recruitment of Clr4 to these sequences and is important  for establishment of silencing.	bind
16280	9	3951	6	11	NULL	NULL	NULL	statement 2	Process		promotes					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2331_s_46	15743828	(B) In contrast, the RNAi-dependent assembly of the RITS complex at  cenH or centromeric sequences promotes recruitment of Clr4 to these sequences and is important  for establishment of silencing.	bind
16281	10	3951	6	11	NULL	NULL	NULL	statement 2	Process		promotes					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2331_s_46	15743828	(B) In contrast, the RNAi-dependent assembly of the RITS complex at  cenH or centromeric sequences promotes recruitment of Clr4 to these sequences and is important  for establishment of silencing.	bind
53775	11	3951	6	11	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2331_s_46	15743828	(B) In contrast, the RNAi-dependent assembly of the RITS complex at  cenH or centromeric sequences promotes recruitment of Clr4 to these sequences and is important  for establishment of silencing.	bind
53780	12	3951	6	11	NULL	NULL	NULL	statement 7	Process		important for					silencing	Process	establishment of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2331_s_46	15743828	(B) In contrast, the RNAi-dependent assembly of the RITS complex at  cenH or centromeric sequences promotes recruitment of Clr4 to these sequences and is important  for establishment of silencing.	bind
53781	13	3951	6	11	NULL	NULL	NULL	statement 8	Process		important for					silencing	Process	establishment of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2331_s_46	15743828	(B) In contrast, the RNAi-dependent assembly of the RITS complex at  cenH or centromeric sequences promotes recruitment of Clr4 to these sequences and is important  for establishment of silencing.	bind
53782	14	3951	6	11	NULL	NULL	NULL	statement 9	Process		important for					silencing	Process	establishment of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2331_s_46	15743828	(B) In contrast, the RNAi-dependent assembly of the RITS complex at  cenH or centromeric sequences promotes recruitment of Clr4 to these sequences and is important  for establishment of silencing.	bind
53783	15	3951	6	11	NULL	NULL	NULL	statement 10	Process		important for					silencing	Process	establishment of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2331_s_46	15743828	(B) In contrast, the RNAi-dependent assembly of the RITS complex at  cenH or centromeric sequences promotes recruitment of Clr4 to these sequences and is important  for establishment of silencing.	bind
9730	1	3952	5	11	NULL	NULL	NULL	HNF4	GP		bind		constitutively			fatty acids	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_2_219_s_36	12191466	(B) In contrast, the work by  Wisely et al. (2002  ) shows that HNF4 constitutively binds fatty acids as structural cofactors, raising the question of how the switch is made from corepressor to coactivator complex.	bind
53883	2	3952	5	11	NULL	NULL	NULL	HNF4	GP		acts as a					structural cofactor	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_2_219_s_36	12191466	(B) In contrast, the work by  Wisely et al. (2002  ) shows that HNF4 constitutively binds fatty acids as structural cofactors, raising the question of how the switch is made from corepressor to coactivator complex.	bind
9572	1	3952	6	11	NULL	NULL	NULL	HNF4	GP		bind		constitutively			fatty acids	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_2_219_s_36	12191466	(B) In contrast, the work by  Wisely et al. (2002  ) shows that HNF4 constitutively binds fatty acids as structural cofactors, raising the question of how the switch is made from corepressor to coactivator complex.	bind
9674	2	3952	6	11	NULL	NULL	NULL	HNF-4	GP		acts as a					structural cofactor	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_2_219_s_36	12191466	(B) In contrast, the work by  Wisely et al. (2002  ) shows that HNF4 constitutively binds fatty acids as structural cofactors, raising the question of how the switch is made from corepressor to coactivator complex.	bind
9731	1	3953	5	11	NULL	NULL	NULL	PP2A 	GP		bind			regulatory B subunit		KSR1	GP				NULL	stimulated cells	NULL	NULL	NULL	NULL	gw60_currbiol_13_16_1356_s_199	12932319	(B) In stimulated cells, Ras activation induces binding of the PP2A regulatory B subunit to the KSR1 and Raf-1 complexes, increasing PP2A activity and resulting in the dephosphorylation of KSR1 on S392 and Raf-1 on S259.	bind
9732	5	3953	5	11	NULL	NULL	NULL	PP2A 	GP		bind			regulatory B subunit		Raf-1 complex	GP				NULL	stimulated cells	NULL	NULL	NULL	NULL	gw60_currbiol_13_16_1356_s_199	12932319	(B) In stimulated cells, Ras activation induces binding of the PP2A regulatory B subunit to the KSR1 and Raf-1 complexes, increasing PP2A activity and resulting in the dephosphorylation of KSR1 on S392 and Raf-1 on S259.	bind
9733	2	3953	5	11	NULL	NULL	NULL	Ras	GP	activation of	induce					statement 1	Process				NULL	stimulated cells	NULL	NULL	NULL	NULL	gw60_currbiol_13_16_1356_s_199	12932319	(B) In stimulated cells, Ras activation induces binding of the PP2A regulatory B subunit to the KSR1 and Raf-1 complexes, increasing PP2A activity and resulting in the dephosphorylation of KSR1 on S392 and Raf-1 on S259.	bind
9734	6	3953	5	11	NULL	NULL	NULL	Ras	GP	activation of	induce					statement 5	Process				NULL	stimulated cells	NULL	NULL	NULL	NULL	gw60_currbiol_13_16_1356_s_199	12932319	(B) In stimulated cells, Ras activation induces binding of the PP2A regulatory B subunit to the KSR1 and Raf-1 complexes, increasing PP2A activity and resulting in the dephosphorylation of KSR1 on S392 and Raf-1 on S259.	bind
9735	3	3953	5	11	NULL	NULL	NULL	statement 2	Process		increase					PP2A	GP	activity of			NULL	stimulated cells	NULL	NULL	NULL	NULL	gw60_currbiol_13_16_1356_s_199	12932319	(B) In stimulated cells, Ras activation induces binding of the PP2A regulatory B subunit to the KSR1 and Raf-1 complexes, increasing PP2A activity and resulting in the dephosphorylation of KSR1 on S392 and Raf-1 on S259.	bind
9736	7	3953	5	11	NULL	NULL	NULL	statement 6	Process		increase					PP2A	GP	activity of			NULL	stimulated cells	NULL	NULL	NULL	NULL	gw60_currbiol_13_16_1356_s_199	12932319	(B) In stimulated cells, Ras activation induces binding of the PP2A regulatory B subunit to the KSR1 and Raf-1 complexes, increasing PP2A activity and resulting in the dephosphorylation of KSR1 on S392 and Raf-1 on S259.	bind
9737	4	3953	5	11	NULL	NULL	NULL	statement 3	Process		results in					KSR1	GP	dephosphorylation of	S392		NULL	stimulated cells	NULL	NULL	NULL	NULL	gw60_currbiol_13_16_1356_s_199	12932319	(B) In stimulated cells, Ras activation induces binding of the PP2A regulatory B subunit to the KSR1 and Raf-1 complexes, increasing PP2A activity and resulting in the dephosphorylation of KSR1 on S392 and Raf-1 on S259.	bind
9738	8	3953	5	11	NULL	NULL	NULL	statement 7	Process		results in					Raf-1	GP	dephosphorylation of	S259		NULL	stimulated cells	NULL	NULL	NULL	NULL	gw60_currbiol_13_16_1356_s_199	12932319	(B) In stimulated cells, Ras activation induces binding of the PP2A regulatory B subunit to the KSR1 and Raf-1 complexes, increasing PP2A activity and resulting in the dephosphorylation of KSR1 on S392 and Raf-1 on S259.	bind
9680	4	3953	6	11	NULL	NULL	NULL	Ras	GP	activation of	dephosphorylates					KSR1	GP		S392		NULL	stimulated cells	NULL	NULL	NULL	NULL	gw60_currbiol_13_16_1356_s_199	12932319	(B) In stimulated cells, Ras activation induces binding of the PP2A regulatory B subunit to the KSR1 and Raf-1 complexes, increasing PP2A activity and resulting in the dephosphorylation of KSR1 on S392 and Raf-1 on S259.	bind
9681	5	3953	6	11	NULL	NULL	NULL	Ras	GP	activation of	dephosphorylates					Raf-1	GP		S259		NULL	stimulated cells	NULL	NULL	NULL	NULL	gw60_currbiol_13_16_1356_s_199	12932319	(B) In stimulated cells, Ras activation induces binding of the PP2A regulatory B subunit to the KSR1 and Raf-1 complexes, increasing PP2A activity and resulting in the dephosphorylation of KSR1 on S392 and Raf-1 on S259.	bind
10497	1	3953	6	11	NULL	NULL	NULL	PP2A	GP		bind			 regulatory B subunit 		KSR1	GP				NULL	stimulated cells	NULL	NULL	NULL	NULL	gw60_currbiol_13_16_1356_s_199	12932319	(B) In stimulated cells, Ras activation induces binding of the PP2A regulatory B subunit to the KSR1 and Raf-1 complexes, increasing PP2A activity and resulting in the dephosphorylation of KSR1 on S392 and Raf-1 on S259.	bind
10498	2	3953	6	11	NULL	NULL	NULL	PP2A 	GP		bind			regulatory B subunit		Raf-1 complexes	GP				NULL	stimulated cells	NULL	NULL	NULL	NULL	gw60_currbiol_13_16_1356_s_199	12932319	(B) In stimulated cells, Ras activation induces binding of the PP2A regulatory B subunit to the KSR1 and Raf-1 complexes, increasing PP2A activity and resulting in the dephosphorylation of KSR1 on S392 and Raf-1 on S259.	bind
10499	3	3953	6	11	NULL	NULL	NULL	statement 1	Process		increases					PP2A	GP	activity of			NULL	stimulated cells	NULL	NULL	NULL	NULL	gw60_currbiol_13_16_1356_s_199	12932319	(B) In stimulated cells, Ras activation induces binding of the PP2A regulatory B subunit to the KSR1 and Raf-1 complexes, increasing PP2A activity and resulting in the dephosphorylation of KSR1 on S392 and Raf-1 on S259.	bind
12505	6	3953	6	11	NULL	NULL	NULL	Ras	GP	activation of	induces					statement 1	Process				NULL	stimulated cells	NULL	NULL	NULL	NULL	gw60_currbiol_13_16_1356_s_199	12932319	(B) In stimulated cells, Ras activation induces binding of the PP2A regulatory B subunit to the KSR1 and Raf-1 complexes, increasing PP2A activity and resulting in the dephosphorylation of KSR1 on S392 and Raf-1 on S259.	bind
53905	7	3953	6	11	NULL	NULL	NULL	statement 2	Process		increases					PP2A	GP	activity of			NULL	stimulated cells	NULL	NULL	NULL	NULL	gw60_currbiol_13_16_1356_s_199	12932319	(B) In stimulated cells, Ras activation induces binding of the PP2A regulatory B subunit to the KSR1 and Raf-1 complexes, increasing PP2A activity and resulting in the dephosphorylation of KSR1 on S392 and Raf-1 on S259.	bind
53906	8	3953	6	11	NULL	NULL	NULL	Ras	GP	activation of	induces					statement 2	Process				NULL	stimulated cells	NULL	NULL	NULL	NULL	gw60_currbiol_13_16_1356_s_199	12932319	(B) In stimulated cells, Ras activation induces binding of the PP2A regulatory B subunit to the KSR1 and Raf-1 complexes, increasing PP2A activity and resulting in the dephosphorylation of KSR1 on S392 and Raf-1 on S259.	bind
9739	1	3954	5	11	NULL	NULL	NULL	CreERT2 	GP		bind					HSP90	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_22_4_430_s_29	12727441	(B) In the absence of appropriate ligand, the CreERT2  fusion protein is bound to the heatshock protein HSP90 and inhibited from entering  the nucleus.	bind
9740	4	3954	5	11	NULL	NULL	NULL	statement 1	Process		in the absence of					appropriate ligand	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_22_4_430_s_29	12727441	(B) In the absence of appropriate ligand, the CreERT2  fusion protein is bound to the heatshock protein HSP90 and inhibited from entering  the nucleus.	bind
9741	2	3954	5	11	NULL	NULL	NULL	CreERT2	GP		is inhibited from					 nucleus	CellComponent	entering into			NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_22_4_430_s_29	12727441	(B) In the absence of appropriate ligand, the CreERT2  fusion protein is bound to the heatshock protein HSP90 and inhibited from entering  the nucleus.	bind
9742	3	3954	5	11	NULL	NULL	NULL	statement 2	Process		occurs following					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_22_4_430_s_29	12727441	(B) In the absence of appropriate ligand, the CreERT2  fusion protein is bound to the heatshock protein HSP90 and inhibited from entering  the nucleus.	bind
53914	5	3954	5	11	NULL	NULL	NULL	HSP90	GP		is a type of					heatshock protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_22_4_430_s_29	12727441	(B) In the absence of appropriate ligand, the CreERT2  fusion protein is bound to the heatshock protein HSP90 and inhibited from entering  the nucleus.	bind
53915	6	3954	5	11	NULL	NULL	NULL	CreERT2	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_22_4_430_s_29	12727441	(B) In the absence of appropriate ligand, the CreERT2  fusion protein is bound to the heatshock protein HSP90 and inhibited from entering  the nucleus.	bind
9573	1	3954	6	11	NULL	NULL	NULL	CreERT2 	GP		bind					 HSP90	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_22_4_430_s_29	12727441	(B) In the absence of appropriate ligand, the CreERT2  fusion protein is bound to the heatshock protein HSP90 and inhibited from entering  the nucleus.	bind
12506	2	3954	6	11	NULL	NULL	NULL	CreERT2	GP		is inhibited from					nucleus	CellComponent	entering into			NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_22_4_430_s_29	12727441	(B) In the absence of appropriate ligand, the CreERT2  fusion protein is bound to the heatshock protein HSP90 and inhibited from entering  the nucleus.	bind
53920	3	3954	6	11	NULL	NULL	NULL	statement 2	Process		occurs following					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_22_4_430_s_29	12727441	(B) In the absence of appropriate ligand, the CreERT2  fusion protein is bound to the heatshock protein HSP90 and inhibited from entering  the nucleus.	bind
53921	4	3954	6	11	NULL	NULL	NULL	statement 1	Process		in the absence of					appropriate ligand	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_22_4_430_s_29	12727441	(B) In the absence of appropriate ligand, the CreERT2  fusion protein is bound to the heatshock protein HSP90 and inhibited from entering  the nucleus.	bind
53922	5	3954	6	11	NULL	NULL	NULL	HSP90	GP		is a type of					heatshock protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_22_4_430_s_29	12727441	(B) In the absence of appropriate ligand, the CreERT2  fusion protein is bound to the heatshock protein HSP90 and inhibited from entering  the nucleus.	bind
53923	6	3954	6	11	NULL	NULL	NULL	CreERT2	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_22_4_430_s_29	12727441	(B) In the absence of appropriate ligand, the CreERT2  fusion protein is bound to the heatshock protein HSP90 and inhibited from entering  the nucleus.	bind
9743	1	3956	5	11	NULL	NULL	NULL	ScaA	GP	enzyme-laden	bind					ScaD	GP	type II cohesins of			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_17_5782_s_193	15317783	(B) In the additional mechanism of attachment, the enzyme-laden ScaA is bound to  the type II cohesins of ScaD, which can also accept a single enzyme via its third  type I cohesin.	bind
9744	2	3956	5	11	NULL	NULL	NULL	ScaD	GP		accept					single enzyme	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_17_5782_s_193	15317783	(B) In the additional mechanism of attachment, the enzyme-laden ScaA is bound to  the type II cohesins of ScaD, which can also accept a single enzyme via its third  type I cohesin.	bind
9745	3	3956	5	11	NULL	NULL	NULL	statement 2	Process		occurs via					 cohesin	GP		third type I		NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_17_5782_s_193	15317783	(B) In the additional mechanism of attachment, the enzyme-laden ScaA is bound to  the type II cohesins of ScaD, which can also accept a single enzyme via its third  type I cohesin.	bind
9574	1	3956	6	11	NULL	NULL	NULL	ScaA	GP	enzyme-laden 	bind					 ScaD	GP	type II cohesins of			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_17_5782_s_193	15317783	(B) In the additional mechanism of attachment, the enzyme-laden ScaA is bound to  the type II cohesins of ScaD, which can also accept a single enzyme via its third  type I cohesin.	bind
12511	2	3956	6	11	NULL	NULL	NULL	ScaD	GP		accept					single enzyme	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_17_5782_s_193	15317783	(B) In the additional mechanism of attachment, the enzyme-laden ScaA is bound to  the type II cohesins of ScaD, which can also accept a single enzyme via its third  type I cohesin.	bind
12512	3	3956	6	11	NULL	NULL	NULL	statement 2	Process		occurs via					cohesin	GP		third type I		NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_17_5782_s_193	15317783	(B) In the additional mechanism of attachment, the enzyme-laden ScaA is bound to  the type II cohesins of ScaD, which can also accept a single enzyme via its third  type I cohesin.	bind
9746	1	3957	5	11	NULL	NULL	NULL	APC	Organism		bind					beta-catenin	GP				NULL	adult colonocyte	NULL	NULL	NULL	NULL	gw60_cellbiol_145_4_699_s_346	10330400	(B) In the adult  colonocyte, Wnt is not present, GSK-3beta activity is constitutively high, and APC binds beta-catenin and targets it for degradation.	bind
9747	2	3957	5	11	NULL	NULL	NULL	statement 1	Process		targets					beta-catenin	GP	 degradation of			NULL	adult colonocyte	NULL	NULL	NULL	NULL	gw60_cellbiol_145_4_699_s_346	10330400	(B) In the adult  colonocyte, Wnt is not present, GSK-3beta activity is constitutively high, and APC binds beta-catenin and targets it for degradation.	bind
53931	3	3957	5	11	NULL	NULL	NULL	Wnt	GP		not present in					adult colonocyte	Cell				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_4_699_s_346	10330400	(B) In the adult  colonocyte, Wnt is not present, GSK-3beta activity is constitutively high, and APC binds beta-catenin and targets it for degradation.	bind
53932	4	3957	5	11	NULL	NULL	NULL	GSK-3beta	GP	activity of	is high in		constitutively			adult colonocyte	Cell				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_4_699_s_346	10330400	(B) In the adult  colonocyte, Wnt is not present, GSK-3beta activity is constitutively high, and APC binds beta-catenin and targets it for degradation.	bind
9575	1	3957	6	11	NULL	NULL	NULL	APC	Organism		bind					beta-catenin	GP				NULL	adult colonocyte	NULL	NULL	NULL	NULL	gw60_cellbiol_145_4_699_s_346	10330400	(B) In the adult  colonocyte, Wnt is not present, GSK-3beta activity is constitutively high, and APC binds beta-catenin and targets it for degradation.	bind
9576	2	3957	6	11	NULL	NULL	NULL	Wnt	GP		is not present in					adult colonocyte	Cell				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_4_699_s_346	10330400	(B) In the adult  colonocyte, Wnt is not present, GSK-3beta activity is constitutively high, and APC binds beta-catenin and targets it for degradation.	bind
9577	3	3957	6	11	NULL	NULL	NULL	GSK-3beta	GP	activity of	is high		constitutively			adult colonocyte	Cell				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_4_699_s_346	10330400	(B) In the adult  colonocyte, Wnt is not present, GSK-3beta activity is constitutively high, and APC binds beta-catenin and targets it for degradation.	bind
53933	4	3957	6	11	NULL	NULL	NULL	statement 1	Process		targets					beta-catenin	GP	degradation of			NULL	adult colonocyte	NULL	NULL	NULL	NULL	gw60_cellbiol_145_4_699_s_346	10330400	(B) In the adult  colonocyte, Wnt is not present, GSK-3beta activity is constitutively high, and APC binds beta-catenin and targets it for degradation.	bind
9748	1	3958	5	11	NULL	NULL	NULL	NT2	GP		bind					Col11a2	GP	WT		promoter sequence	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4256_s_236	12024037	(B) In the left panel, lane 2 shows that NT2 bound to the WT  Col11a2 promoter sequence.	bind
9578	1	3958	6	11	NULL	NULL	NULL	NT2	GP		bind					Col11a2	GP	wild type		promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4256_s_236	12024037	(B) In the left panel, lane 2 shows that NT2 bound to the WT  Col11a2 promoter sequence.	bind
9749	1	3959	5	11	NULL	NULL	NULL	transposase	GP		forms complex with					transposon	GP		end fragments		NULL		NULL	NULL	NULL	NULL	gw60_cell_84_2_223_s_64	8565068	(B) In the presence of IHF, transposase builds a synaptic  complex with a pair of transposon end fragments (paired ends complex or  PEC;  Sakai et al., 1995   ).	bind
9750	2	3959	5	11	NULL	NULL	NULL	statement 1	Process		in the presence of					IHF	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_84_2_223_s_64	8565068	(B) In the presence of IHF, transposase builds a synaptic  complex with a pair of transposon end fragments (paired ends complex or  PEC;  Sakai et al., 1995   ).	bind
53934	3	3959	5	11	NULL	NULL	NULL	statement 1	Process		forms					synaptic complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_84_2_223_s_64	8565068	(B) In the presence of IHF, transposase builds a synaptic  complex with a pair of transposon end fragments (paired ends complex or  PEC;  Sakai et al., 1995   ).	bind
53935	4	3959	5	11	NULL	NULL	NULL	PEC	GP		is					paired ends complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_84_2_223_s_64	8565068	(B) In the presence of IHF, transposase builds a synaptic  complex with a pair of transposon end fragments (paired ends complex or  PEC;  Sakai et al., 1995   ).	bind
9579	1	3959	6	11	NULL	NULL	NULL	transposase	GP		forms a complex with					transposon	GP		end fragments		NULL		NULL	NULL	NULL	NULL	gw60_cell_84_2_223_s_64	8565068	(B) In the presence of IHF, transposase builds a synaptic  complex with a pair of transposon end fragments (paired ends complex or  PEC;  Sakai et al., 1995   ).	bind
9580	2	3959	6	11	NULL	NULL	NULL	PEC	GP		is					paired ends complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_84_2_223_s_64	8565068	(B) In the presence of IHF, transposase builds a synaptic  complex with a pair of transposon end fragments (paired ends complex or  PEC;  Sakai et al., 1995   ).	bind
9581	3	3959	6	11	NULL	NULL	NULL	statement 1	Process		occurs in presence of					IHF	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_84_2_223_s_64	8565068	(B) In the presence of IHF, transposase builds a synaptic  complex with a pair of transposon end fragments (paired ends complex or  PEC;  Sakai et al., 1995   ).	bind
53936	4	3959	6	11	NULL	NULL	NULL	statement 1	Process		forms					synaptic complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_84_2_223_s_64	8565068	(B) In the presence of IHF, transposase builds a synaptic  complex with a pair of transposon end fragments (paired ends complex or  PEC;  Sakai et al., 1995   ).	bind
9751	1	3960	5	11	NULL	NULL	NULL	WAK1	GP		bind					OEE2	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_305_4_862_s_127	12767910	(B) In vitro binding of  WAK1 to OEE2.	bind
9582	1	3960	6	11	NULL	NULL	NULL	WAK1	GP		bind					OEE2	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_305_4_862_s_127	12767910	(B) In vitro binding of  WAK1 to OEE2.	bind
9752	1	3961	5	11	NULL	NULL	NULL	ASAP1b	GP		bind					GST-Src	GP		SH3		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7038_s_327	9819391	(B) In vitro binding of ASAP1b to GST-Src SH3 and GST-Crk.	bind
9753	2	3961	5	11	NULL	NULL	NULL	ASAP1b	GP		bind					GST-Crk	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7038_s_327	9819391	(B) In vitro binding of ASAP1b to GST-Src SH3 and GST-Crk.	bind
9583	1	3961	6	11	NULL	NULL	NULL	 ASAP1b	GP		bind					GST-Src	GP		SH3 domain		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7038_s_327	9819391	(B) In vitro binding of ASAP1b to GST-Src SH3 and GST-Crk.	bind
9584	2	3961	6	11	NULL	NULL	NULL	ASAP1b	GP		bind					GST-Crk	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7038_s_327	9819391	(B) In vitro binding of ASAP1b to GST-Src SH3 and GST-Crk.	bind
9754	1	3962	5	11	NULL	NULL	NULL	E2F	GP		bind					PPAR 1	GP			promoter	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_devcell_3_1_39_s_70	12110166	(B) In vitro binding of E2F to the  PPAR 1 promoter.	bind
9585	1	3962	6	11	NULL	NULL	NULL	E2F	GP		bind					PPAR1	GP			promoter	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_devcell_3_1_39_s_70	12110166	(B) In vitro binding of E2F to the  PPAR 1 promoter.	bind
9755	1	3963	5	11	NULL	NULL	NULL	Gab1	GP		bind			MBD		Met	GP	WT			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcell_7_6_1293_s_35	11430831	(B) In vitro binding of Gab1, Grb2, Src, and p85PI3K by MetWT and Metd. GST-fusion proteins of the Gab1 Met binding domain (MBD), the carboxyl-terminal p85PI3K SH2, the Src SH2, and full size Grb2 were immobilized on glutathione-Sepharose and incubated with lysates of untreated or HGF-stimulated  metWT/WT and  metd/d hepatocytes.	bind
9756	2	3963	5	11	NULL	NULL	NULL	Gab1	GP		bind			MBD		Metd	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcell_7_6_1293_s_35	11430831	(B) In vitro binding of Gab1, Grb2, Src, and p85PI3K by MetWT and Metd. GST-fusion proteins of the Gab1 Met binding domain (MBD), the carboxyl-terminal p85PI3K SH2, the Src SH2, and full size Grb2 were immobilized on glutathione-Sepharose and incubated with lysates of untreated or HGF-stimulated  metWT/WT and  metd/d hepatocytes.	bind
9757	3	3963	5	11	NULL	NULL	NULL	Grb2	GP	full size	bind					Met	GP	WT			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcell_7_6_1293_s_35	11430831	(B) In vitro binding of Gab1, Grb2, Src, and p85PI3K by MetWT and Metd. GST-fusion proteins of the Gab1 Met binding domain (MBD), the carboxyl-terminal p85PI3K SH2, the Src SH2, and full size Grb2 were immobilized on glutathione-Sepharose and incubated with lysates of untreated or HGF-stimulated  metWT/WT and  metd/d hepatocytes.	bind
9758	4	3963	5	11	NULL	NULL	NULL	Grb2	GP	full size	bind					Metd	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcell_7_6_1293_s_35	11430831	(B) In vitro binding of Gab1, Grb2, Src, and p85PI3K by MetWT and Metd. GST-fusion proteins of the Gab1 Met binding domain (MBD), the carboxyl-terminal p85PI3K SH2, the Src SH2, and full size Grb2 were immobilized on glutathione-Sepharose and incubated with lysates of untreated or HGF-stimulated  metWT/WT and  metd/d hepatocytes.	bind
9759	5	3963	5	11	NULL	NULL	NULL	Src	GP		bind			SH2		Met	GP	WT			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcell_7_6_1293_s_35	11430831	(B) In vitro binding of Gab1, Grb2, Src, and p85PI3K by MetWT and Metd. GST-fusion proteins of the Gab1 Met binding domain (MBD), the carboxyl-terminal p85PI3K SH2, the Src SH2, and full size Grb2 were immobilized on glutathione-Sepharose and incubated with lysates of untreated or HGF-stimulated  metWT/WT and  metd/d hepatocytes.	bind
9760	6	3963	5	11	NULL	NULL	NULL	Src	GP		bind			SH2		Metd	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcell_7_6_1293_s_35	11430831	(B) In vitro binding of Gab1, Grb2, Src, and p85PI3K by MetWT and Metd. GST-fusion proteins of the Gab1 Met binding domain (MBD), the carboxyl-terminal p85PI3K SH2, the Src SH2, and full size Grb2 were immobilized on glutathione-Sepharose and incubated with lysates of untreated or HGF-stimulated  metWT/WT and  metd/d hepatocytes.	bind
9761	7	3963	5	11	NULL	NULL	NULL	p85PI3K	GP		bind			carboxyl-terminal;;SH2		Met	GP	WT			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcell_7_6_1293_s_35	11430831	(B) In vitro binding of Gab1, Grb2, Src, and p85PI3K by MetWT and Metd. GST-fusion proteins of the Gab1 Met binding domain (MBD), the carboxyl-terminal p85PI3K SH2, the Src SH2, and full size Grb2 were immobilized on glutathione-Sepharose and incubated with lysates of untreated or HGF-stimulated  metWT/WT and  metd/d hepatocytes.	bind
9762	8	3963	5	11	NULL	NULL	NULL	p85PI3K	GP		bind			 carboxyl-terminal;;SH2		Metd	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcell_7_6_1293_s_35	11430831	(B) In vitro binding of Gab1, Grb2, Src, and p85PI3K by MetWT and Metd. GST-fusion proteins of the Gab1 Met binding domain (MBD), the carboxyl-terminal p85PI3K SH2, the Src SH2, and full size Grb2 were immobilized on glutathione-Sepharose and incubated with lysates of untreated or HGF-stimulated  metWT/WT and  metd/d hepatocytes.	bind
53971	9	3963	5	11	NULL	NULL	NULL	MBD	GP		is					Met binding domain	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_6_1293_s_35	11430831	(B) In vitro binding of Gab1, Grb2, Src, and p85PI3K by MetWT and Metd. GST-fusion proteins of the Gab1 Met binding domain (MBD), the carboxyl-terminal p85PI3K SH2, the Src SH2, and full size Grb2 were immobilized on glutathione-Sepharose and incubated with lysates of untreated or HGF-stimulated  metWT/WT and  metd/d hepatocytes.	bind
9682	1	3963	6	11	NULL	NULL	NULL	Gab1	GP		bind			MBD		Met	GP	wild type			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcell_7_6_1293_s_35	11430831	(B) In vitro binding of Gab1, Grb2, Src, and p85PI3K by MetWT and Metd. GST-fusion proteins of the Gab1 Met binding domain (MBD), the carboxyl-terminal p85PI3K SH2, the Src SH2, and full size Grb2 were immobilized on glutathione-Sepharose and incubated with lysates of untreated or HGF-stimulated  metWT/WT and  metd/d hepatocytes.	bind
9683	2	3963	6	11	NULL	NULL	NULL	Gab1	GP		bind			MBD		Metd	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_6_1293_s_35	11430831	(B) In vitro binding of Gab1, Grb2, Src, and p85PI3K by MetWT and Metd. GST-fusion proteins of the Gab1 Met binding domain (MBD), the carboxyl-terminal p85PI3K SH2, the Src SH2, and full size Grb2 were immobilized on glutathione-Sepharose and incubated with lysates of untreated or HGF-stimulated  metWT/WT and  metd/d hepatocytes.	bind
9684	3	3963	6	11	NULL	NULL	NULL	Grb2	GP	full size	bind					Met	GP	wild type			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcell_7_6_1293_s_35	11430831	(B) In vitro binding of Gab1, Grb2, Src, and p85PI3K by MetWT and Metd. GST-fusion proteins of the Gab1 Met binding domain (MBD), the carboxyl-terminal p85PI3K SH2, the Src SH2, and full size Grb2 were immobilized on glutathione-Sepharose and incubated with lysates of untreated or HGF-stimulated  metWT/WT and  metd/d hepatocytes.	bind
9685	4	3963	6	11	NULL	NULL	NULL	Grb2	GP	full size	bind					Metd	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcell_7_6_1293_s_35	11430831	(B) In vitro binding of Gab1, Grb2, Src, and p85PI3K by MetWT and Metd. GST-fusion proteins of the Gab1 Met binding domain (MBD), the carboxyl-terminal p85PI3K SH2, the Src SH2, and full size Grb2 were immobilized on glutathione-Sepharose and incubated with lysates of untreated or HGF-stimulated  metWT/WT and  metd/d hepatocytes.	bind
9686	5	3963	6	11	NULL	NULL	NULL	MBD	GP		is					Met binding domain	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_6_1293_s_35	11430831	(B) In vitro binding of Gab1, Grb2, Src, and p85PI3K by MetWT and Metd. GST-fusion proteins of the Gab1 Met binding domain (MBD), the carboxyl-terminal p85PI3K SH2, the Src SH2, and full size Grb2 were immobilized on glutathione-Sepharose and incubated with lysates of untreated or HGF-stimulated  metWT/WT and  metd/d hepatocytes.	bind
9687	6	3963	6	11	NULL	NULL	NULL	Src	GP		bind			SH2 domain		Met	GP	wild type			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcell_7_6_1293_s_35	11430831	(B) In vitro binding of Gab1, Grb2, Src, and p85PI3K by MetWT and Metd. GST-fusion proteins of the Gab1 Met binding domain (MBD), the carboxyl-terminal p85PI3K SH2, the Src SH2, and full size Grb2 were immobilized on glutathione-Sepharose and incubated with lysates of untreated or HGF-stimulated  metWT/WT and  metd/d hepatocytes.	bind
9688	7	3963	6	11	NULL	NULL	NULL	Src	GP		bind			SH2 domain		Metd	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcell_7_6_1293_s_35	11430831	(B) In vitro binding of Gab1, Grb2, Src, and p85PI3K by MetWT and Metd. GST-fusion proteins of the Gab1 Met binding domain (MBD), the carboxyl-terminal p85PI3K SH2, the Src SH2, and full size Grb2 were immobilized on glutathione-Sepharose and incubated with lysates of untreated or HGF-stimulated  metWT/WT and  metd/d hepatocytes.	bind
9689	8	3963	6	11	NULL	NULL	NULL	p85PI3K	GP		bind			carboxyl-terminal domain;;SH2		Met	GP	wild type			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcell_7_6_1293_s_35	11430831	(B) In vitro binding of Gab1, Grb2, Src, and p85PI3K by MetWT and Metd. GST-fusion proteins of the Gab1 Met binding domain (MBD), the carboxyl-terminal p85PI3K SH2, the Src SH2, and full size Grb2 were immobilized on glutathione-Sepharose and incubated with lysates of untreated or HGF-stimulated  metWT/WT and  metd/d hepatocytes.	bind
9690	9	3963	6	11	NULL	NULL	NULL	p85PI3K	GP		bind			carboxyl-terminal domain;;SH2		Metd	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcell_7_6_1293_s_35	11430831	(B) In vitro binding of Gab1, Grb2, Src, and p85PI3K by MetWT and Metd. GST-fusion proteins of the Gab1 Met binding domain (MBD), the carboxyl-terminal p85PI3K SH2, the Src SH2, and full size Grb2 were immobilized on glutathione-Sepharose and incubated with lysates of untreated or HGF-stimulated  metWT/WT and  metd/d hepatocytes.	bind
9763	1	3964	5	11	NULL	NULL	NULL	h411/414	GP		bind					RanBP3	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8751_s_270	14612415	(B) In vitro binding of h411/414 to RanBP3.	bind
9586	1	3964	6	11	NULL	NULL	NULL	h411/414	GP		bind					RanBP3	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8751_s_270	14612415	(B) In vitro binding of h411/414 to RanBP3.	bind
9764	1	3965	5	11	NULL	NULL	NULL	Siah-1	GP		bind					Sina protein	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_724_s_176	9858595	(B) In vitro binding of Siah-1 to the Sina protein.	bind
9587	1	3965	6	11	NULL	NULL	NULL	Siah-1	GP		bind					Sina protein	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_724_s_176	9858595	(B) In vitro binding of Siah-1 to the Sina protein.	bind
9765	1	3966	5	11	NULL	NULL	NULL	Numb	GP		bind			PTB domain		Nak	GP		C terminus		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_598_s_143	9418906	(B) In vitro binding of the Numb PTB domain to the Nak C terminus.	bind
9588	1	3966	6	11	NULL	NULL	NULL	Numb	GP		bind			PTB domain		Nak	GP		C terminus		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_598_s_143	9418906	(B) In vitro binding of the Numb PTB domain to the Nak C terminus.	bind
9766	1	3967	5	11	NULL	NULL	NULL	titin	GP		bind					obscurin	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_cellbiol_154_1_123_s_175	11448995	(B) In vitro binding of titin to obscurin.	bind
9589	1	3967	6	11	NULL	NULL	NULL	titin	GP		bind					obscurin	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_cellbiol_154_1_123_s_175	11448995	(B) In vitro binding of titin to obscurin.	bind
9767	1	3968	5	11	NULL	NULL	NULL	WAK1	GP		bind					OEE2	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_305_4_862_s_127	12767910	(B) In vitro binding of WAK1 to OEE2.	bind
9590	1	3968	6	11	NULL	NULL	NULL	WAK1	GP		bind					OEE2	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_305_4_862_s_127	12767910	(B) In vitro binding of WAK1 to OEE2.	bind
9768	1	3970	5	11	NULL	NULL	NULL	NF-kB	GP		bind					DNA	NucleicAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_2957_s_266	15798185	(B) In vitro DNA binding assay of NF-kB.	bind
9591	1	3970	6	11	NULL	NULL	NULL	NF-kB	GP		bind					DNA	NucleicAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_2957_s_266	15798185	(B) In vitro DNA binding assay of NF-kB.	bind
9769	1	3971	5	11	NULL	NULL	NULL	Miz-1	GP		bind					GST-TopBP1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcell_10_3_509_s_71	12408820	(B) In vitro GST binding assays demonstrating POZ-dependent binding of Miz-1 to GST-TopBP1 but not to GST alone.	bind
9770	2	3971	5	11	NULL	NULL	NULL	Miz-1	GP		does not bind					GST	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcell_10_3_509_s_71	12408820	(B) In vitro GST binding assays demonstrating POZ-dependent binding of Miz-1 to GST-TopBP1 but not to GST alone.	bind
9771	3	3971	5	11	NULL	NULL	NULL	statement 1	Process		is dependent on								POZ		NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_3_509_s_71	12408820	(B) In vitro GST binding assays demonstrating POZ-dependent binding of Miz-1 to GST-TopBP1 but not to GST alone.	bind
9592	1	3971	6	11	NULL	NULL	NULL	Miz-1	GP		bind					GST-TopBP1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_3_509_s_71	12408820	(B) In vitro GST binding assays demonstrating POZ-dependent binding of Miz-1 to GST-TopBP1 but not to GST alone.	bind
9593	2	3971	6	11	NULL	NULL	NULL	statement 1	Process		is dependent on								POZ		NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_3_509_s_71	12408820	(B) In vitro GST binding assays demonstrating POZ-dependent binding of Miz-1 to GST-TopBP1 but not to GST alone.	bind
9594	3	3971	6	11	NULL	NULL	NULL	Miz-1	GP		does not bind					GST	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_3_509_s_71	12408820	(B) In vitro GST binding assays demonstrating POZ-dependent binding of Miz-1 to GST-TopBP1 but not to GST alone.	bind
9772	1	3974	5	11	NULL	NULL	NULL	Adaptin protein	GP	in vitro-translated	bind					GST-Numb	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_2_221_s_161	12194853	(B) In vitro-translated  -Adaptin protein binds GST-Numb, but binding to GST-Numb 5  (Frise et al., 1996  ) lacking amino acids (aa) 426-546 is strongly reduced.	bind
9773	2	3974	5	11	NULL	NULL	NULL	Adaptin protein	GP	in vitro-translated	bind					GST-Numb 5	GP	lacking amino acids	426-546		NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_2_221_s_161	12194853	(B) In vitro-translated  -Adaptin protein binds GST-Numb, but binding to GST-Numb 5  (Frise et al., 1996  ) lacking amino acids (aa) 426-546 is strongly reduced.	bind
9774	3	3974	5	11	NULL	NULL	NULL	statement 2	Process	binding of	reduced than		strongly			statement 1	Process	binding of			NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_2_221_s_161	12194853	(B) In vitro-translated  -Adaptin protein binds GST-Numb, but binding to GST-Numb 5  (Frise et al., 1996  ) lacking amino acids (aa) 426-546 is strongly reduced.	bind
9595	1	3974	6	11	NULL	NULL	NULL	Adaptin protein	GP	in vitro-translated	bind					GST-Numb 5	GP	lacking amino acids	426-546		NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_2_221_s_161	12194853	(B) In vitro-translated  -Adaptin protein binds GST-Numb, but binding to GST-Numb 5  (Frise et al., 1996  ) lacking amino acids (aa) 426-546 is strongly reduced.	bind
16267	2	3974	6	11	NULL	NULL	NULL	Adaptin protein	GP	in vitro-translated	bind					GST-Numb	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_2_221_s_161	12194853	(B) In vitro-translated  -Adaptin protein binds GST-Numb, but binding to GST-Numb 5  (Frise et al., 1996  ) lacking amino acids (aa) 426-546 is strongly reduced.	bind
16276	3	3974	6	11	NULL	NULL	NULL	statement 2	Process	binding of	reduced than		strongly			statement 1	Process	binding of			NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_2_221_s_161	12194853	(B) In vitro-translated  -Adaptin protein binds GST-Numb, but binding to GST-Numb 5  (Frise et al., 1996  ) lacking amino acids (aa) 426-546 is strongly reduced.	bind
9775	1	3977	5	11	NULL	NULL	NULL	IRF-1	GP		bind					IL-4	GP			promoter	NULL	in vivo Jurkat T cells transfected with IRF-1 expression vectors	NULL	NULL	NULL	NULL	gw60_immunity_17_6_703_s_186	12479817	(B) In vivo binding of IRF-1 and IRF-2 to the IL-4 promoter was assessed by ChIP with Jurkat T cells transfected with IRF-1 and IRF-2 expression vectors.	bind
9776	2	3977	5	11	NULL	NULL	NULL	IRF-2	GP		bind					IL-4	GP			promoter	NULL	in vivo Jurkat T cells transfected with IRF-2 expression vectors	NULL	NULL	NULL	NULL	gw60_immunity_17_6_703_s_186	12479817	(B) In vivo binding of IRF-1 and IRF-2 to the IL-4 promoter was assessed by ChIP with Jurkat T cells transfected with IRF-1 and IRF-2 expression vectors.	bind
9777	1	3977	6	11	NULL	NULL	NULL	IRF-1	GP		bind					IL-4	GP			promoter	NULL	Jurkat T cells transfected with  IRF-1 expression vector	NULL	NULL	NULL	NULL	gw60_immunity_17_6_703_s_186	12479817	(B) In vivo binding of IRF-1 and IRF-2 to the IL-4 promoter was assessed by ChIP with Jurkat T cells transfected with IRF-1 and IRF-2 expression vectors.	bind
9778	1	3978	5	11	NULL	NULL	NULL	MEK5 protein sequences	GP		bind					ERK5	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_6_2065_s_71	16507987	(B) In vivo binding of MEK5 protein sequences and ERK5.	bind
9782	1	3978	6	11	NULL	NULL	NULL	MEK5 protein sequences	GP		bind					ERK5	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_6_2065_s_71	16507987	(B) In vivo binding of MEK5 protein sequences and ERK5.	bind
9780	1	3979	5	11	NULL	NULL	NULL	GTP	Chemical		bind					Ras	GP				NULL	transiently transfected NIH 3T3 cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4611_s_271	10373510	(B) In vivo measurement of GTP and GDP bound to Ras in transiently transfected NIH 3T3 cells.	bind
9781	2	3979	5	11	NULL	NULL	NULL	GDP	Chemical		bind					Ras	GP				NULL	transiently transfected NIH 3T3 cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4611_s_271	10373510	(B) In vivo measurement of GTP and GDP bound to Ras in transiently transfected NIH 3T3 cells.	bind
9783	1	3979	6	11	NULL	NULL	NULL	GTP	Chemical		bind					Ras	GP				NULL	transiently transfected NIH 3T3 cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4611_s_271	10373510	(B) In vivo measurement of GTP and GDP bound to Ras in transiently transfected NIH 3T3 cells.	bind
9784	2	3979	6	11	NULL	NULL	NULL	GDP	Chemical		bind					Ras	GP				NULL	transiently transfected NIH 3T3 cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4611_s_271	10373510	(B) In vivo measurement of GTP and GDP bound to Ras in transiently transfected NIH 3T3 cells.	bind
9789	1	3981	5	11	NULL	NULL	NULL	Nck-1	GP		bind			SH3(1)		GST-IRE1alpha	GP	bound to glutathione-Sepharose beads			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_9_4248_s_200	15201339	(B) Individual SH3 domains of  Nck-1, Nck-1-SH3(1), Nck-1-SH3(2), and Nck-1-SH3(3), fused to GST were cleaved with  thrombin, GST and thrombin were depleted and the products were pulled down with GST-IRE1alpha or GST-IRE1beta bound to glutathione-Sepharose beads.	bind
9790	2	3981	5	11	NULL	NULL	NULL	Nck-1	GP		bind			SH3(1)		GST-IRE1beta	GP	bound to glutathione-Sepharose beads			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_9_4248_s_200	15201339	(B) Individual SH3 domains of  Nck-1, Nck-1-SH3(1), Nck-1-SH3(2), and Nck-1-SH3(3), fused to GST were cleaved with  thrombin, GST and thrombin were depleted and the products were pulled down with GST-IRE1alpha or GST-IRE1beta bound to glutathione-Sepharose beads.	bind
9791	3	3981	5	11	NULL	NULL	NULL	Nck-1	GP		bind			SH3(2)		GST-IRE1alpha	GP	bound to glutathione-Sepharose beads			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_9_4248_s_200	15201339	(B) Individual SH3 domains of  Nck-1, Nck-1-SH3(1), Nck-1-SH3(2), and Nck-1-SH3(3), fused to GST were cleaved with  thrombin, GST and thrombin were depleted and the products were pulled down with GST-IRE1alpha or GST-IRE1beta bound to glutathione-Sepharose beads.	bind
9792	4	3981	5	11	NULL	NULL	NULL	Nck-1	GP		bind			SH3(2)		GST-IRE1beta	GP	bound to glutathione-Sepharose beads			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_9_4248_s_200	15201339	(B) Individual SH3 domains of  Nck-1, Nck-1-SH3(1), Nck-1-SH3(2), and Nck-1-SH3(3), fused to GST were cleaved with  thrombin, GST and thrombin were depleted and the products were pulled down with GST-IRE1alpha or GST-IRE1beta bound to glutathione-Sepharose beads.	bind
9794	5	3981	5	11	NULL	NULL	NULL	Nck-1	GP		bind			SH3(3)		GST-IRE1alpha	GP	bound to glutathione-Sepharose beads			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_9_4248_s_200	15201339	(B) Individual SH3 domains of  Nck-1, Nck-1-SH3(1), Nck-1-SH3(2), and Nck-1-SH3(3), fused to GST were cleaved with  thrombin, GST and thrombin were depleted and the products were pulled down with GST-IRE1alpha or GST-IRE1beta bound to glutathione-Sepharose beads.	bind
9795	6	3981	5	11	NULL	NULL	NULL	Nck-1	GP		bind			SH3(3)		GST-IRE1beta	GP	bound to glutathione-Sepharose beads			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_9_4248_s_200	15201339	(B) Individual SH3 domains of  Nck-1, Nck-1-SH3(1), Nck-1-SH3(2), and Nck-1-SH3(3), fused to GST were cleaved with  thrombin, GST and thrombin were depleted and the products were pulled down with GST-IRE1alpha or GST-IRE1beta bound to glutathione-Sepharose beads.	bind
9779	2	3981	6	11	NULL	NULL	NULL	IRF-2	GP		bind					IL-4	GP			promoter	NULL	Jurkat T cells transfected with  IRF-2 expression vector	NULL	NULL	NULL	NULL	gw70_molbiolcell_15_9_4248_s_200	15201339	(B) Individual SH3 domains of  Nck-1, Nck-1-SH3(1), Nck-1-SH3(2), and Nck-1-SH3(3), fused to GST were cleaved with  thrombin, GST and thrombin were depleted and the products were pulled down with GST-IRE1alpha or GST-IRE1beta bound to glutathione-Sepharose beads.	bind
9785	1	3981	6	11	NULL	NULL	NULL	GST-IRE1alpha	GP		bind					NCk-1	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_9_4248_s_200	15201339	(B) Individual SH3 domains of  Nck-1, Nck-1-SH3(1), Nck-1-SH3(2), and Nck-1-SH3(3), fused to GST were cleaved with  thrombin, GST and thrombin were depleted and the products were pulled down with GST-IRE1alpha or GST-IRE1beta bound to glutathione-Sepharose beads.	bind
9786	2	3981	6	11	NULL	NULL	NULL	GST-IRE1beta	GP		bind					NCk-1	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_9_4248_s_200	15201339	(B) Individual SH3 domains of  Nck-1, Nck-1-SH3(1), Nck-1-SH3(2), and Nck-1-SH3(3), fused to GST were cleaved with  thrombin, GST and thrombin were depleted and the products were pulled down with GST-IRE1alpha or GST-IRE1beta bound to glutathione-Sepharose beads.	bind
9787	3	3981	6	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_9_4248_s_200	15201339	(B) Individual SH3 domains of  Nck-1, Nck-1-SH3(1), Nck-1-SH3(2), and Nck-1-SH3(3), fused to GST were cleaved with  thrombin, GST and thrombin were depleted and the products were pulled down with GST-IRE1alpha or GST-IRE1beta bound to glutathione-Sepharose beads.	bind
9797	1	3982	5	11	NULL	NULL	NULL	IRFs	GP		bind					IL-4	GP			IRF binding sites	NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_6_703_s_101	12479817	(B) Inducible binding of IRFs to the IL-4 IRF binding sites upon IFN-  stimulation.	bind
9798	2	3982	5	11	NULL	NULL	NULL	IFN	GP	stimulation	induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_6_703_s_101	12479817	(B) Inducible binding of IRFs to the IL-4 IRF binding sites upon IFN-  stimulation.	bind
9788	1	3982	6	11	NULL	NULL	NULL	IRFs	GP		bind					IL-4	GP			IRF binding site	NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_6_703_s_101	12479817	(B) Inducible binding of IRFs to the IL-4 IRF binding sites upon IFN-  stimulation.	bind
9793	2	3982	6	11	NULL	NULL	NULL	IFN	GP	stimulation of	induces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_6_703_s_101	12479817	(B) Inducible binding of IRFs to the IL-4 IRF binding sites upon IFN-  stimulation.	bind
9799	1	3983	5	11	NULL	NULL	NULL	PpsR	GP		bind					puc	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_cell_110_5_613_s_170	12230978	(B) Influence of light on PpsR binding to a  puc promoter probe.	bind
9796	1	3983	6	11	NULL	NULL	NULL	PpsR	GP		bind					puc	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_cell_110_5_613_s_170	12230978	(B) Influence of light on PpsR binding to a  puc promoter probe.	bind
9800	1	3985	5	11	NULL	NULL	NULL	Pit1	GP		inhibit					GATA2	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_cell_97_5_587_s_134	10367888	(B) Inhibition of  GATA2 binding by Pit1.	bind
9813	1	3985	6	11	NULL	NULL	NULL	Pit1	GP		inhibits					GATA2	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_cell_97_5_587_s_134	10367888	(B) Inhibition of  GATA2 binding by Pit1.	bind
9801	1	3986	5	11	NULL	NULL	NULL	125I- -bungarotoxin 	Chemical		bind					SH-SY5Y-h 7 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_13_2533_s_191	11044725	(B) Inhibition of 125I- -bungarotoxin ( -BTx) binding to SH-SY5Y-h 7 cells by verapamil.	bind
9802	2	3986	5	11	NULL	NULL	NULL	verapamil	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_13_2533_s_191	11044725	(B) Inhibition of 125I- -bungarotoxin ( -BTx) binding to SH-SY5Y-h 7 cells by verapamil.	bind
54012	3	3986	5	11	NULL	NULL	NULL	BTx	Chemical		is					bungarotoxin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_13_2533_s_191	11044725	(B) Inhibition of 125I- -bungarotoxin ( -BTx) binding to SH-SY5Y-h 7 cells by verapamil.	bind
9817	1	3986	6	11	NULL	NULL	NULL	125I- -bungarotoxin	Chemical		bind					SH-SY5Y-h 7 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_13_2533_s_191	11044725	(B) Inhibition of 125I- -bungarotoxin ( -BTx) binding to SH-SY5Y-h 7 cells by verapamil.	bind
9819	2	3986	6	11	NULL	NULL	NULL	BTx	Chemical		is					bungarotoxin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_13_2533_s_191	11044725	(B) Inhibition of 125I- -bungarotoxin ( -BTx) binding to SH-SY5Y-h 7 cells by verapamil.	bind
9820	3	3986	6	11	NULL	NULL	NULL	verapamil	Chemical		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_13_2533_s_191	11044725	(B) Inhibition of 125I- -bungarotoxin ( -BTx) binding to SH-SY5Y-h 7 cells by verapamil.	bind
9803	1	3987	5	11	NULL	NULL	NULL	FKHR	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_1_104_s_255	12482965	(B) Inhibition of FKHR DNA binding by activated androgen receptor.	bind
9804	2	3987	5	11	NULL	NULL	NULL	androgen receptor	GP	activated	inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_1_104_s_255	12482965	(B) Inhibition of FKHR DNA binding by activated androgen receptor.	bind
9827	1	3987	6	11	NULL	NULL	NULL	FKHR	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_1_104_s_255	12482965	(B) Inhibition of FKHR DNA binding by activated androgen receptor.	bind
9828	2	3987	6	11	NULL	NULL	NULL	androgen receptor	GP	activated	inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_1_104_s_255	12482965	(B) Inhibition of FKHR DNA binding by activated androgen receptor.	bind
9805	1	3988	5	11	NULL	NULL	NULL	Hgl2	GP	cysteine-rich	bind		specifically			GalNAc19BSA	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_8_3836_s_175	10417146	(b) Inhibition of GalNAc-specific binding of cysteine-rich Hgl2 to GalNAc19BSA with asialofetuin (ASF) and holotransferrin (hT) at 25 or 50 muM.	bind
9807	2	3988	5	11	NULL	NULL	NULL	ASF	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_8_3836_s_175	10417146	(b) Inhibition of GalNAc-specific binding of cysteine-rich Hgl2 to GalNAc19BSA with asialofetuin (ASF) and holotransferrin (hT) at 25 or 50 muM.	bind
9808	3	3988	5	11	NULL	NULL	NULL	ASF	GP		is					asialofetuin	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_8_3836_s_175	10417146	(b) Inhibition of GalNAc-specific binding of cysteine-rich Hgl2 to GalNAc19BSA with asialofetuin (ASF) and holotransferrin (hT) at 25 or 50 muM.	bind
9809	4	3988	5	11	NULL	NULL	NULL	hT	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_8_3836_s_175	10417146	(b) Inhibition of GalNAc-specific binding of cysteine-rich Hgl2 to GalNAc19BSA with asialofetuin (ASF) and holotransferrin (hT) at 25 or 50 muM.	bind
9810	5	3988	5	11	NULL	NULL	NULL	hT	GP		is					holotransferrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_8_3836_s_175	10417146	(b) Inhibition of GalNAc-specific binding of cysteine-rich Hgl2 to GalNAc19BSA with asialofetuin (ASF) and holotransferrin (hT) at 25 or 50 muM.	bind
9829	1	3988	6	11	NULL	NULL	NULL	Hgl2	GP	cysteine-rich	bind		specifically			GalNAc19BSA	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_8_3836_s_175	10417146	(b) Inhibition of GalNAc-specific binding of cysteine-rich Hgl2 to GalNAc19BSA with asialofetuin (ASF) and holotransferrin (hT) at 25 or 50 muM.	bind
9830	2	3988	6	11	NULL	NULL	NULL	ASF	GP		is					asialofetuin	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_8_3836_s_175	10417146	(b) Inhibition of GalNAc-specific binding of cysteine-rich Hgl2 to GalNAc19BSA with asialofetuin (ASF) and holotransferrin (hT) at 25 or 50 muM.	bind
9831	3	3988	6	11	NULL	NULL	NULL	hT	GP		is					holotransferrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_8_3836_s_175	10417146	(b) Inhibition of GalNAc-specific binding of cysteine-rich Hgl2 to GalNAc19BSA with asialofetuin (ASF) and holotransferrin (hT) at 25 or 50 muM.	bind
9832	4	3988	6	11	NULL	NULL	NULL	ASF	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_8_3836_s_175	10417146	(b) Inhibition of GalNAc-specific binding of cysteine-rich Hgl2 to GalNAc19BSA with asialofetuin (ASF) and holotransferrin (hT) at 25 or 50 muM.	bind
9833	5	3988	6	11	NULL	NULL	NULL	hT	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_8_3836_s_175	10417146	(b) Inhibition of GalNAc-specific binding of cysteine-rich Hgl2 to GalNAc19BSA with asialofetuin (ASF) and holotransferrin (hT) at 25 or 50 muM.	bind
9811	1	3989	5	11	NULL	NULL	NULL	H-2	GP	biotinylated	bind			N-terminal		EF-Tu	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_chembiol_10_2_161_s_101	12618188	(B) Inhibition of N-terminal biotinylated  H-2 (0.5  M) binding to immobilized EF-Tu by N-terminal acetylated  H-2.	bind
9812	2	3989	5	11	NULL	NULL	NULL	H-2	GP	acetylated	inhibit			N-terminal		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_10_2_161_s_101	12618188	(B) Inhibition of N-terminal biotinylated  H-2 (0.5  M) binding to immobilized EF-Tu by N-terminal acetylated  H-2.	bind
9834	1	3989	6	11	NULL	NULL	NULL	H-2	GP	biotinylated	bind			N-terminus		EF-Tu	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_chembiol_10_2_161_s_101	12618188	(B) Inhibition of N-terminal biotinylated  H-2 (0.5  M) binding to immobilized EF-Tu by N-terminal acetylated  H-2.	bind
9835	2	3989	6	11	NULL	NULL	NULL	H-2	GP	acetylated	inhibits			N-terminal 		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_10_2_161_s_101	12618188	(B) Inhibition of N-terminal biotinylated  H-2 (0.5  M) binding to immobilized EF-Tu by N-terminal acetylated  H-2.	bind
9814	1	3990	5	11	NULL	NULL	NULL	peptide V	GP		mediate					HDL	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_4_753_s_290	10191300	(B) Inhibition of peptide V-mediated binding of HDL by HDL, LDL, and AcLDL.	bind
9815	2	3990	5	11	NULL	NULL	NULL	HDL	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_4_753_s_290	10191300	(B) Inhibition of peptide V-mediated binding of HDL by HDL, LDL, and AcLDL.	bind
9816	3	3990	5	11	NULL	NULL	NULL	LDL	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_4_753_s_290	10191300	(B) Inhibition of peptide V-mediated binding of HDL by HDL, LDL, and AcLDL.	bind
9818	4	3990	5	11	NULL	NULL	NULL	AcLDL	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_4_753_s_290	10191300	(B) Inhibition of peptide V-mediated binding of HDL by HDL, LDL, and AcLDL.	bind
9836	1	3990	6	11	NULL	NULL	NULL	peptide V	GP		mediates					HDL	Chemical	binding of 			NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_4_753_s_290	10191300	(B) Inhibition of peptide V-mediated binding of HDL by HDL, LDL, and AcLDL.	bind
9837	2	3990	6	11	NULL	NULL	NULL	HDL	Chemical		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_4_753_s_290	10191300	(B) Inhibition of peptide V-mediated binding of HDL by HDL, LDL, and AcLDL.	bind
9838	3	3990	6	11	NULL	NULL	NULL	LDL	Chemical		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_4_753_s_290	10191300	(B) Inhibition of peptide V-mediated binding of HDL by HDL, LDL, and AcLDL.	bind
9839	4	3990	6	11	NULL	NULL	NULL	AcLDL	Chemical		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_4_753_s_290	10191300	(B) Inhibition of peptide V-mediated binding of HDL by HDL, LDL, and AcLDL.	bind
9821	1	3991	5	11	NULL	NULL	NULL	GTP	Chemical		bind					Rac	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_161_2_381_s_167	12707308	(B) Inhibition of ROCK activity in the presence of high concentration of  SDF-1alpha (500 ng/ml) increases the GTP-bound form of Rac.	bind
9822	2	3991	5	11	NULL	NULL	NULL	SDF-1alpha	GP	high concentration of	inhibit					ROCK	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_161_2_381_s_167	12707308	(B) Inhibition of ROCK activity in the presence of high concentration of  SDF-1alpha (500 ng/ml) increases the GTP-bound form of Rac.	bind
9823	3	3991	5	11	NULL	NULL	NULL	statement 2	Process		increase					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_161_2_381_s_167	12707308	(B) Inhibition of ROCK activity in the presence of high concentration of  SDF-1alpha (500 ng/ml) increases the GTP-bound form of Rac.	bind
9921	1	3991	6	11	NULL	NULL	NULL	GTP	Chemical		bind					Rac	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_161_2_381_s_167	12707308	(B) Inhibition of ROCK activity in the presence of high concentration of  SDF-1alpha (500 ng/ml) increases the GTP-bound form of Rac.	bind
9922	2	3991	6	11	NULL	NULL	NULL	ROCK activity	GP	inhibition of	increases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_161_2_381_s_167	12707308	(B) Inhibition of ROCK activity in the presence of high concentration of  SDF-1alpha (500 ng/ml) increases the GTP-bound form of Rac.	bind
9923	3	3991	6	11	NULL	NULL	NULL	statement 2	Process		occurs in presence of					SDF-1 alpha	GP	high concentration of			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_161_2_381_s_167	12707308	(B) Inhibition of ROCK activity in the presence of high concentration of  SDF-1alpha (500 ng/ml) increases the GTP-bound form of Rac.	bind
9824	1	3993	5	11	NULL	NULL	NULL	GR 113808	Chemical		bind		specifically			h5-HT4(n) receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_42_1_60_s_174	11750916	(B) Inhibition of specific [3]GR 113808 binding to h5-HT4(n) receptors.	bind
9841	1	3993	6	11	NULL	NULL	NULL	GR 113808	Chemical		bind		specifically			h5-HT4(n) receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_42_1_60_s_174	11750916	(B) Inhibition of specific [3]GR 113808 binding to h5-HT4(n) receptors.	bind
9825	1	3994	5	11	NULL	NULL	NULL	TnrA	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_4_427_s_54	11719184	(B) Inhibition of TnrA DNA binding by GS  in the presence and absence of feedback  inhibitors.	bind
9826	2	3994	5	11	NULL	NULL	NULL	GS	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_4_427_s_54	11719184	(B) Inhibition of TnrA DNA binding by GS  in the presence and absence of feedback  inhibitors.	bind
9844	1	3994	6	11	NULL	NULL	NULL	TnrA	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_4_427_s_54	11719184	(B) Inhibition of TnrA DNA binding by GS  in the presence and absence of feedback  inhibitors.	bind
9845	2	3994	6	11	NULL	NULL	NULL	GS	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_4_427_s_54	11719184	(B) Inhibition of TnrA DNA binding by GS  in the presence and absence of feedback  inhibitors.	bind
9842	1	3995	5	11	NULL	NULL	NULL	Syk-NC-SH2	GP		bind					Fc RII	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1451_2_353_s_110	10556589	(B) Inhibitory effect of peptides corresponding to ITAM on the binding of Syk-NC-SH2 to Fc RII.	bind
9843	2	3995	5	11	NULL	NULL	NULL	ITAM peptides	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1451_2_353_s_110	10556589	(B) Inhibitory effect of peptides corresponding to ITAM on the binding of Syk-NC-SH2 to Fc RII.	bind
9846	1	3995	6	11	NULL	NULL	NULL	Syk-NC-SH2	GP		bind					Fc-RII	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1451_2_353_s_110	10556589	(B) Inhibitory effect of peptides corresponding to ITAM on the binding of Syk-NC-SH2 to Fc RII.	bind
9847	2	3995	6	11	NULL	NULL	NULL	ITAM peptides	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1451_2_353_s_110	10556589	(B) Inhibitory effect of peptides corresponding to ITAM on the binding of Syk-NC-SH2 to Fc RII.	bind
9890	1	3996	5	11	NULL	NULL	NULL	GTP S	Chemical		bind					KA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_38_7_991_s_111	10428417	(B) Intracellular Ca2+ was required for attenuation of DPDPE-stimulated [35]GTP S binding by KA or PMA.	bind
9891	2	3996	5	11	NULL	NULL	NULL	GTP S	Chemical		bind					PMA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_38_7_991_s_111	10428417	(B) Intracellular Ca2+ was required for attenuation of DPDPE-stimulated [35]GTP S binding by KA or PMA.	bind
9892	3	3996	5	11	NULL	NULL	NULL	DPDPE	Chemical		stimulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_38_7_991_s_111	10428417	(B) Intracellular Ca2+ was required for attenuation of DPDPE-stimulated [35]GTP S binding by KA or PMA.	bind
9893	4	3996	5	11	NULL	NULL	NULL	DPDPE	Chemical		stimulate					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_38_7_991_s_111	10428417	(B) Intracellular Ca2+ was required for attenuation of DPDPE-stimulated [35]GTP S binding by KA or PMA.	bind
9894	5	3996	5	11	NULL	NULL	NULL	Ca2+	Chemical	intracellular	attenuate					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_38_7_991_s_111	10428417	(B) Intracellular Ca2+ was required for attenuation of DPDPE-stimulated [35]GTP S binding by KA or PMA.	bind
9895	6	3996	5	11	NULL	NULL	NULL	Ca2+	Chemical	intracellular	attenuate					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_38_7_991_s_111	10428417	(B) Intracellular Ca2+ was required for attenuation of DPDPE-stimulated [35]GTP S binding by KA or PMA.	bind
54017	7	3996	5	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_38_7_991_s_111	10428417	(B) Intracellular Ca2+ was required for attenuation of DPDPE-stimulated [35]GTP S binding by KA or PMA.	bind
9848	1	3996	6	11	NULL	NULL	NULL	GTP S	Chemical		bind					KA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_38_7_991_s_111	10428417	(B) Intracellular Ca2+ was required for attenuation of DPDPE-stimulated [35]GTP S binding by KA or PMA.	bind
9849	2	3996	6	11	NULL	NULL	NULL	GTP S	Chemical		bind					PMA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_38_7_991_s_111	10428417	(B) Intracellular Ca2+ was required for attenuation of DPDPE-stimulated [35]GTP S binding by KA or PMA.	bind
9850	3	3996	6	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_38_7_991_s_111	10428417	(B) Intracellular Ca2+ was required for attenuation of DPDPE-stimulated [35]GTP S binding by KA or PMA.	bind
9851	4	3996	6	11	NULL	NULL	NULL	DPDPE	Chemical		stimulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_38_7_991_s_111	10428417	(B) Intracellular Ca2+ was required for attenuation of DPDPE-stimulated [35]GTP S binding by KA or PMA.	bind
9852	5	3996	6	11	NULL	NULL	NULL	DPDPE	Chemical		stimulates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_38_7_991_s_111	10428417	(B) Intracellular Ca2+ was required for attenuation of DPDPE-stimulated [35]GTP S binding by KA or PMA.	bind
9853	6	3996	6	11	NULL	NULL	NULL	Intracellular Ca2+	Chemical		attenuates					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_38_7_991_s_111	10428417	(B) Intracellular Ca2+ was required for attenuation of DPDPE-stimulated [35]GTP S binding by KA or PMA.	bind
9854	7	3996	6	11	NULL	NULL	NULL	Intracellular Ca2+	Chemical		attenuates					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_38_7_991_s_111	10428417	(B) Intracellular Ca2+ was required for attenuation of DPDPE-stimulated [35]GTP S binding by KA or PMA.	bind
9840	1	3998	5	11	NULL	NULL	NULL	IRF-1	GP		bind					mu	NucleicAcid			enhancer	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_11_6870_s_212	9774700	(B) IRF-1 binding to the mu enhancer.	bind
9855	1	3998	6	11	NULL	NULL	NULL	IRF-1	GP		bind					mu	NucleicAcid			enhancer	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_11_6870_s_212	9774700	(B) IRF-1 binding to the mu enhancer.	bind
9896	1	4000	5	11	NULL	NULL	NULL	JNK	GP		bind					MKK7beta	GP		NH2 terminus		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_2_1569_s_185	9891090	(B) JNK binds to the NH2 terminus of MKK7beta.	bind
9856	1	4000	6	11	NULL	NULL	NULL	JNK	GP		bind					MKK7beta	GP		NH2 terminus		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_2_1569_s_185	9891090	(B) JNK binds to the NH2 terminus of MKK7beta.	bind
9897	1	4001	5	11	NULL	NULL	NULL	p34/p20 complex	GP		bind					ADP-Pi	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_5_1041_s_166	11741539	(B) Kd measurements for p34/p20 and Arp2/3 complex binding to ADP-Pi and ADP F-actin.	bind
9898	2	4001	5	11	NULL	NULL	NULL	p34/p20 complex	GP		bind					ADP F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_5_1041_s_166	11741539	(B) Kd measurements for p34/p20 and Arp2/3 complex binding to ADP-Pi and ADP F-actin.	bind
9899	3	4001	5	11	NULL	NULL	NULL	Arp2/3 complex	GP		bind					ADP-Pi	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_5_1041_s_166	11741539	(B) Kd measurements for p34/p20 and Arp2/3 complex binding to ADP-Pi and ADP F-actin.	bind
9900	4	4001	5	11	NULL	NULL	NULL	Arp2/3 complex	GP		bind					ADP F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_5_1041_s_166	11741539	(B) Kd measurements for p34/p20 and Arp2/3 complex binding to ADP-Pi and ADP F-actin.	bind
12173	1	4001	7	11	NULL	NULL	NULL	p34/p20 complex	GP		bind					ADP-Pi	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_5_1041_s_166	11741539	(B) Kd measurements for p34/p20 and Arp2/3 complex binding to ADP-Pi and ADP F-actin.	bind
12174	2	4001	7	11	NULL	NULL	NULL	p34/p20 complex	GP		bind					ADP F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_5_1041_s_166	11741539	(B) Kd measurements for p34/p20 and Arp2/3 complex binding to ADP-Pi and ADP F-actin.	bind
12175	3	4001	7	11	NULL	NULL	NULL	Arp2/3 complex	GP		bind					 ADP-Pi	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_5_1041_s_166	11741539	(B) Kd measurements for p34/p20 and Arp2/3 complex binding to ADP-Pi and ADP F-actin.	bind
12176	4	4001	7	11	NULL	NULL	NULL	Arp2/3 complex	GP		bind					ADP F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_5_1041_s_166	11741539	(B) Kd measurements for p34/p20 and Arp2/3 complex binding to ADP-Pi and ADP F-actin.	bind
9901	1	4003	5	11	NULL	NULL	NULL	Syt 1	GP		does not bind					GST-NECAB 	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_112_1_51_s_150	12044471	(B) Lack of binding of Syt 1 and Mint 2 to GST-NECAB fusion proteins.	bind
9902	2	4003	5	11	NULL	NULL	NULL	Mint 2	GP		does not bind					GST-NECAB	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_112_1_51_s_150	12044471	(B) Lack of binding of Syt 1 and Mint 2 to GST-NECAB fusion proteins.	bind
44538	3	4003	5	11	NULL	NULL	NULL	GST-NECAB	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_112_1_51_s_150	12044471	(B) Lack of binding of Syt 1 and Mint 2 to GST-NECAB fusion proteins.	bind
12177	1	4003	7	11	NULL	NULL	NULL	Syt 1	GP		does not bind					 GST-NECAB	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_112_1_51_s_150	12044471	(B) Lack of binding of Syt 1 and Mint 2 to GST-NECAB fusion proteins.	bind
12178	2	4003	7	11	NULL	NULL	NULL	Mint 2	GP		does not bind					GST-NECAB	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_112_1_51_s_150	12044471	(B) Lack of binding of Syt 1 and Mint 2 to GST-NECAB fusion proteins.	bind
44404	3	4003	7	11	NULL	NULL	NULL	GST-NECAB	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_112_1_51_s_150	12044471	(B) Lack of binding of Syt 1 and Mint 2 to GST-NECAB fusion proteins.	bind
9903	1	4004	5	11	NULL	NULL	NULL	Shc	GP		does not bind					TrkB receptors	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_2_335_s_74	9728915	(B) Lack of Shc binding to mutant TrkB receptors.	bind
12179	1	4004	7	11	NULL	NULL	NULL	Shc	GP		does not bind					TrkB receptor	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_2_335_s_74	9728915	(B) Lack of Shc binding to mutant TrkB receptors.	bind
10077	1	4006	5	11	NULL	NULL	NULL	Top2p	GP		bind									CEN4 region	NULL		NULL	NULL	NULL	NULL	gw70_genetics_172_2_783_s_108	16204216	(B) Layout of the PCR probes used for ChIP analysis of Top2p binding to the  CEN4 region.	bind
12180	1	4006	7	11	NULL	NULL	NULL	Top2p	GP		bind									CEN4 region	NULL		NULL	NULL	NULL	NULL	gw70_genetics_172_2_783_s_108	16204216	(B) Layout of the PCR probes used for ChIP analysis of Top2p binding to the  CEN4 region.	bind
10078	1	4008	5	11	NULL	NULL	NULL	Lef1	GP		bind					Brn-2	GP			promoter	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_7_2915_s_100	15024079	(B) Lef1 binds the  Brn-2 promoter in vitro.	bind
12181	1	4008	7	11	NULL	NULL	NULL	Lef1	GP		bind					Brn-2 	GP			promoter	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_7_2915_s_100	15024079	(B) Lef1 binds the  Brn-2 promoter in vitro.	bind
10079	1	4009	5	11	NULL	NULL	NULL	TAFII250	GP	in vitro-expressed	bind					GST	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_846_s_128	9858607	(B) Levels of in vitro-expressed TAFII250 bound to GST, TBP, or Rb, as detected by Western analysis (monoclonal anti-hTAFII250 antibody) of nonradioactive, duplicate kinase reactions performed concurrently with those shown in panel A.	bind
10080	2	4009	5	11	NULL	NULL	NULL	TAFII250	GP	in vitro-expressed	bind					TBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_846_s_128	9858607	(B) Levels of in vitro-expressed TAFII250 bound to GST, TBP, or Rb, as detected by Western analysis (monoclonal anti-hTAFII250 antibody) of nonradioactive, duplicate kinase reactions performed concurrently with those shown in panel A.	bind
10081	3	4009	5	11	NULL	NULL	NULL	TAFII250	GP	in vitro-expressed	bind					Rb	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_846_s_128	9858607	(B) Levels of in vitro-expressed TAFII250 bound to GST, TBP, or Rb, as detected by Western analysis (monoclonal anti-hTAFII250 antibody) of nonradioactive, duplicate kinase reactions performed concurrently with those shown in panel A.	bind
12182	1	4009	7	11	NULL	NULL	NULL	TAFII250	GP	in vitro-expressed	bind					GST	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_846_s_128	9858607	(B) Levels of in vitro-expressed TAFII250 bound to GST, TBP, or Rb, as detected by Western analysis (monoclonal anti-hTAFII250 antibody) of nonradioactive, duplicate kinase reactions performed concurrently with those shown in panel A.	bind
12183	2	4009	7	11	NULL	NULL	NULL	TAFII250	GP	in vitro-expressed	bind					TBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_846_s_128	9858607	(B) Levels of in vitro-expressed TAFII250 bound to GST, TBP, or Rb, as detected by Western analysis (monoclonal anti-hTAFII250 antibody) of nonradioactive, duplicate kinase reactions performed concurrently with those shown in panel A.	bind
12184	3	4009	7	11	NULL	NULL	NULL	TAFII250	GP	in vitro-expressed	bind					Rb	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_846_s_128	9858607	(B) Levels of in vitro-expressed TAFII250 bound to GST, TBP, or Rb, as detected by Western analysis (monoclonal anti-hTAFII250 antibody) of nonradioactive, duplicate kinase reactions performed concurrently with those shown in panel A.	bind
10082	1	4010	5	11	NULL	NULL	NULL	Snapin	GP		bind					GST-SNAP23	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_3_1245_s_359	15635093	(B) Likewise, inhibition of Snapin binding to GST-SNAP23 (10 mug)  was determined in the presence of EBAG9.	bind
10083	2	4010	5	11	NULL	NULL	NULL	EBAG9	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_3_1245_s_359	15635093	(B) Likewise, inhibition of Snapin binding to GST-SNAP23 (10 mug)  was determined in the presence of EBAG9.	bind
12185	1	4010	7	11	NULL	NULL	NULL	Snapin	GP		bind					GST-SNAP23	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_3_1245_s_359	15635093	(B) Likewise, inhibition of Snapin binding to GST-SNAP23 (10 mug)  was determined in the presence of EBAG9.	bind
12186	2	4010	7	11	NULL	NULL	NULL	EBAG9	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_3_1245_s_359	15635093	(B) Likewise, inhibition of Snapin binding to GST-SNAP23 (10 mug)  was determined in the presence of EBAG9.	bind
10086	1	4012	5	11	NULL	NULL	NULL	peptides	amino acid	proline-rich	is derived from					C3G	GP		Crk-binding region		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_5_3044_s_172	9566923	(B) Linker insertion mutations in the Crk SH3 domain disrupt binding to proline-rich peptides derived from the Crk-binding region of C3G.	bind
10087	2	4012	5	11	NULL	NULL	NULL	Crk	GP		bind			SH3 domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_5_3044_s_172	9566923	(B) Linker insertion mutations in the Crk SH3 domain disrupt binding to proline-rich peptides derived from the Crk-binding region of C3G.	bind
10088	3	4012	5	11	NULL	NULL	NULL	Crk	GP	linker insertion mutations in	disrupt			SH3 domain		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_5_3044_s_172	9566923	(B) Linker insertion mutations in the Crk SH3 domain disrupt binding to proline-rich peptides derived from the Crk-binding region of C3G.	bind
12262	1	4012	7	11	NULL	NULL	NULL	 Crk	GP		bind			SH3		 peptides	amino acid	proline-rich			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_5_3044_s_172	9566923	(B) Linker insertion mutations in the Crk SH3 domain disrupt binding to proline-rich peptides derived from the Crk-binding region of C3G.	bind
12263	2	4012	7	11	NULL	NULL	NULL	Crk	GP	Linker insertion mutations in	disrupt			SH3 domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_5_3044_s_172	9566923	(B) Linker insertion mutations in the Crk SH3 domain disrupt binding to proline-rich peptides derived from the Crk-binding region of C3G.	bind
12264	3	4012	7	11	NULL	NULL	NULL	proline-rich peptide	amino acid		is derived from					C3G	GP		Crk-binding region of		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_5_3044_s_172	9566923	(B) Linker insertion mutations in the Crk SH3 domain disrupt binding to proline-rich peptides derived from the Crk-binding region of C3G.	bind
10089	1	4013	5	11	NULL	NULL	NULL	GTP	Chemical		bind					Rheb	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_6_1457_s_54	12820960	(B) Loss of TSC2 function leads to elevated levels of GTP bound Rheb.	bind
10090	2	4013	5	11	NULL	NULL	NULL	TSC2	GP	loss of 	leads to					statement 1	Process	elevated levels of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_6_1457_s_54	12820960	(B) Loss of TSC2 function leads to elevated levels of GTP bound Rheb.	bind
12265	1	4013	7	11	NULL	NULL	NULL	GTP	Chemical		bind					Rheb	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_6_1457_s_54	12820960	(B) Loss of TSC2 function leads to elevated levels of GTP bound Rheb.	bind
12266	2	4013	7	11	NULL	NULL	NULL	TSC2	GP	Loss of	leads to					statement 1	Process	elevated levels of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_6_1457_s_54	12820960	(B) Loss of TSC2 function leads to elevated levels of GTP bound Rheb.	bind
10091	1	4014	5	11	NULL	NULL	NULL	MAb 24c5	GP		bind					GC	Chemical	dilute concentrations of 			NULL	in M. tuberculosis	NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_143	11953397	(B) MAb 24c5 binding to dilute concentrations of GC in the  M. tuberculosis GC ELISA.	bind
12267	1	4014	7	11	NULL	NULL	NULL	MAb 24c5	GP		bind					GC	Chemical	dilute concentrations of			NULL	M. tuberculosis	NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_143	11953397	(B) MAb 24c5 binding to dilute concentrations of GC in the  M. tuberculosis GC ELISA.	bind
10092	1	4020	5	11	NULL	NULL	NULL	JAK	GP		bind					AT1aR	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9829_s_210	16260600	(B) Maximal AII-induced ANF transactivation  requires JAK binding to AT1aR.	bind
10093	2	4020	5	11	NULL	NULL	NULL	Maximal AII	GP		induce					ANF	GP	transactivation of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9829_s_210	16260600	(B) Maximal AII-induced ANF transactivation  requires JAK binding to AT1aR.	bind
10094	3	4020	5	11	NULL	NULL	NULL	statement 2	Process		require					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9829_s_210	16260600	(B) Maximal AII-induced ANF transactivation  requires JAK binding to AT1aR.	bind
12468	1	4020	7	11	NULL	NULL	NULL	JAK	GP		bind					AT1aR	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9829_s_210	16260600	(B) Maximal AII-induced ANF transactivation  requires JAK binding to AT1aR.	bind
12469	2	4020	7	11	NULL	NULL	NULL	Maximal AII	GP		induce					ANF	GP	transactivation of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9829_s_210	16260600	(B) Maximal AII-induced ANF transactivation  requires JAK binding to AT1aR.	bind
12470	3	4020	7	11	NULL	NULL	NULL	statement 2	Process		requires					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9829_s_210	16260600	(B) Maximal AII-induced ANF transactivation  requires JAK binding to AT1aR.	bind
10095	1	4021	5	11	NULL	NULL	NULL	MBP	GP		does not bind					F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_130_18_4427_s_138	12900458	(B) MBP does not bind  to F-actin.	bind
12471	1	4021	7	11	NULL	NULL	NULL	MBP	GP		does not bind					F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_130_18_4427_s_138	12900458	(B) MBP does not bind  to F-actin.	bind
10097	1	4023	5	11	NULL	NULL	NULL	Mbp-Ndt80	GP	E. coli	bind					MSE	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_5_685_s_176	9660952	(B) Mbp-Ndt80 isolated from  E. colibinds the MSE.	bind
12472	1	4023	7	11	NULL	NULL	NULL	Mbp-Ndt80	GP	E.coli	bind					MSE	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_5_685_s_176	9660952	(B) Mbp-Ndt80 isolated from  E. colibinds the MSE.	bind
10099	1	4026	5	11	NULL	NULL	NULL	Mediator complex	GP		contains					CDK8	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_14_4604_s_175	11416138	(B) Mediator complexes containing CDK8 and cyclin C are bound by the VDR LBD.	bind
10100	2	4026	5	11	NULL	NULL	NULL	Mediator complex	GP		contains					cyclin C	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_14_4604_s_175	11416138	(B) Mediator complexes containing CDK8 and cyclin C are bound by the VDR LBD.	bind
10101	3	4026	5	11	NULL	NULL	NULL	VDR	GP		bind			LBD		statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_14_4604_s_175	11416138	(B) Mediator complexes containing CDK8 and cyclin C are bound by the VDR LBD.	bind
10102	4	4026	5	11	NULL	NULL	NULL	VDR	GP		bind			LBD		statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_14_4604_s_175	11416138	(B) Mediator complexes containing CDK8 and cyclin C are bound by the VDR LBD.	bind
12478	1	4026	7	11	NULL	NULL	NULL	mediator complex	GP		bind					VDR	GP		LBD		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_14_4604_s_175	11416138	(B) Mediator complexes containing CDK8 and cyclin C are bound by the VDR LBD.	bind
12479	2	4026	7	11	NULL	NULL	NULL	mediator complex	GP		bind					VDR	GP		LBD		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_14_4604_s_175	11416138	(B) Mediator complexes containing CDK8 and cyclin C are bound by the VDR LBD.	bind
12480	3	4026	7	11	NULL	NULL	NULL	mediator complex	GP		contain					CDK8	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_14_4604_s_175	11416138	(B) Mediator complexes containing CDK8 and cyclin C are bound by the VDR LBD.	bind
12481	4	4026	7	11	NULL	NULL	NULL	mediator complex	GP		contain					cyclin C	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_14_4604_s_175	11416138	(B) Mediator complexes containing CDK8 and cyclin C are bound by the VDR LBD.	bind
10103	1	4027	5	11	NULL	NULL	NULL	GRP1	GP		bind			PH domain		PtdIns-3,4,5-P3	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_160_1_89_s_138	12507995	(B) Membrane recruitment of the PtdIns-3,4,5-P3 - binding PH domain of GRP1.	bind
10104	2	4027	5	11	NULL	NULL	NULL	statement 1	GP		is recruited to					membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_160_1_89_s_138	12507995	(B) Membrane recruitment of the PtdIns-3,4,5-P3 - binding PH domain of GRP1.	bind
12482	2	4027	7	11	NULL	NULL	NULL	statement 1	GP		is recruited to					membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_160_1_89_s_138	12507995	(B) Membrane recruitment of the PtdIns-3,4,5-P3 - binding PH domain of GRP1.	bind
44405	1	4027	7	11	NULL	NULL	NULL	GRP1	GP		bind			PH domain		PtdIns-3,4,5-P3	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_160_1_89_s_138	12507995	(B) Membrane recruitment of the PtdIns-3,4,5-P3 - binding PH domain of GRP1.	bind
10105	1	4028	5	11	NULL	NULL	NULL	Methoprene	Chemical		bind					dUSP	GP				NULL		NULL	NULL	NULL	NULL	gw60_insectbiochemmolbiol_32_1_33_s_233	11719067	(B) Methoprene (40  M) binds to dUSP and causes suppression in fluorescence.	bind
12483	1	4028	7	11	NULL	NULL	NULL	Methoprene	Chemical		bind					dUSP	GP				NULL		NULL	NULL	NULL	NULL	gw60_insectbiochemmolbiol_32_1_33_s_233	11719067	(B) Methoprene (40  M) binds to dUSP and causes suppression in fluorescence.	bind
10107	1	4030	5	11	NULL	NULL	NULL	MIM	GP		bind					F-actin	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_cellbiol_168_3_453_s_118	15684034	(B) MIM binds F-actin  in vitro .	bind
12484	1	4030	7	11	NULL	NULL	NULL	MIM	GP		bind					F-actin	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_cellbiol_168_3_453_s_118	15684034	(B) MIM binds F-actin  in vitro .	bind
10108	1	4031	5	11	NULL	NULL	NULL	 p97	GP	mitotically phosphorylated	bind					p47	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_161_6_1067_s_146	12810701	(B) Mitotically phosphorylated  p97 binds to p47.	bind
12485	1	4031	7	11	NULL	NULL	NULL	 p97	GP	mitotically phosphorylated	bind					p47	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_161_6_1067_s_146	12810701	(B) Mitotically phosphorylated  p97 binds to p47.	bind
10109	1	4032	5	11	NULL	NULL	NULL	p97	GP	mitotically phosphorylated	bind					p47	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_161_6_1067_s_145	12810701	(B) Mitotically phosphorylated p97 binds to p47.	bind
10110	1	4033	5	11	NULL	NULL	NULL	Mlc2p	GP		bind					Myo1p	GP		IQ2		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_165_6_843_s_80	15210731	(B) Mlc2p  binds to Myo1p through IQ2.	bind
12486	1	4033	7	11	NULL	NULL	NULL	Mlc2p	GP		bind					Myo1p	GP		IQ2		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_165_6_843_s_80	15210731	(B) Mlc2p  binds to Myo1p through IQ2.	bind
10112	1	4035	5	11	NULL	NULL	NULL	ZEBRA	GP		bind									Z-3 binding site	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_375	10825199	(B) Model depicting how HMG-1 induces cooperative binding of ZEBRA to the Z-3 and Z-4 pair of binding sites.	bind
10113	2	4035	5	11	NULL	NULL	NULL	ZEBRA	GP		bind									Z-4 binding site	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_375	10825199	(B) Model depicting how HMG-1 induces cooperative binding of ZEBRA to the Z-3 and Z-4 pair of binding sites.	bind
10114	3	4035	5	11	NULL	NULL	NULL	statement 1	Process		occurs in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_375	10825199	(B) Model depicting how HMG-1 induces cooperative binding of ZEBRA to the Z-3 and Z-4 pair of binding sites.	bind
10115	4	4035	5	11	NULL	NULL	NULL	HMG-1	GP		induce					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_375	10825199	(B) Model depicting how HMG-1 induces cooperative binding of ZEBRA to the Z-3 and Z-4 pair of binding sites.	bind
12487	1	4035	7	11	NULL	NULL	NULL	ZEBRA	GP		bind									Z-3 binding site	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_375	10825199	(B) Model depicting how HMG-1 induces cooperative binding of ZEBRA to the Z-3 and Z-4 pair of binding sites.	bind
12488	2	4035	7	11	NULL	NULL	NULL	ZEBRA	GP		bind								 	Z-4 binding site	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_375	10825199	(B) Model depicting how HMG-1 induces cooperative binding of ZEBRA to the Z-3 and Z-4 pair of binding sites.	bind
12489	3	4035	7	11	NULL	NULL	NULL	statement 1	Process		occurs in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_375	10825199	(B) Model depicting how HMG-1 induces cooperative binding of ZEBRA to the Z-3 and Z-4 pair of binding sites.	bind
12490	4	4035	7	11	NULL	NULL	NULL	HMG-1	GP		induces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_375	10825199	(B) Model depicting how HMG-1 induces cooperative binding of ZEBRA to the Z-3 and Z-4 pair of binding sites.	bind
12491	5	4035	7	11	NULL	NULL	NULL	HMG-1	GP		induces					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_375	10825199	(B) Model depicting how HMG-1 induces cooperative binding of ZEBRA to the Z-3 and Z-4 pair of binding sites.	bind
10116	1	4036	5	11	NULL	NULL	NULL	snapin	GP		bind					cypin	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_11_5103_s_291	16120643	(B) Model for snapin and  tubulin binding to cypin.	bind
10117	2	4036	5	11	NULL	NULL	NULL	tubulin	GP		bind					cypin	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_11_5103_s_291	16120643	(B) Model for snapin and  tubulin binding to cypin.	bind
12492	1	4036	7	11	NULL	NULL	NULL	snapin	GP		bind					cypin	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_11_5103_s_291	16120643	(B) Model for snapin and  tubulin binding to cypin.	bind
12493	2	4036	7	11	NULL	NULL	NULL	tubulin	GP		bind					cypin	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_11_5103_s_291	16120643	(B) Model for snapin and  tubulin binding to cypin.	bind
10118	1	4037	5	11	NULL	NULL	NULL	Mot3	GP		bind					Ty912delta	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_1879_s_271	9528759	(B) Mot3 binding to the  Ty912delta promoter is zinc dependent.	bind
10119	2	4037	5	11	NULL	NULL	NULL	statement 1	Process		is dependent on					zinc	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_1879_s_271	9528759	(B) Mot3 binding to the  Ty912delta promoter is zinc dependent.	bind
12494	1	4037	7	11	NULL	NULL	NULL	Mot3	GP		bind					Ty912delta	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_1879_s_271	9528759	(B) Mot3 binding to the  Ty912delta promoter is zinc dependent.	bind
12495	2	4037	7	11	NULL	NULL	NULL	statement 1	Process		is dependent on					zinc	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_1879_s_271	9528759	(B) Mot3 binding to the  Ty912delta promoter is zinc dependent.	bind
10120	1	4038	5	11	NULL	NULL	NULL	mSin3A	GP		bind								ETO domains		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6470_s_205	11533236	(B) mSin3A and N-CoR bind to distinct ETO domains.	bind
10121	2	4038	5	11	NULL	NULL	NULL	N-CoR	GP		bind								ETO domains		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6470_s_205	11533236	(B) mSin3A and N-CoR bind to distinct ETO domains.	bind
12496	1	4038	7	11	NULL	NULL	NULL	mSin3A	GP		bind								ETO domain		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6470_s_205	11533236	(B) mSin3A and N-CoR bind to distinct ETO domains.	bind
12497	2	4038	7	11	NULL	NULL	NULL	Nn-CoR	GP		bind								ETO domain		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6470_s_205	11533236	(B) mSin3A and N-CoR bind to distinct ETO domains.	bind
10122	1	4039	5	11	NULL	NULL	NULL	MSP	GP		bind					VAB-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_132_23_5225_s_383	16267094	(B) MSP binding to VAB-1 triggers a switch (SW) from  negative to positive regulation.	bind
10123	3	4039	5	11	NULL	NULL	NULL	statement 1	Process		triggers					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_132_23_5225_s_383	16267094	(B) MSP binding to VAB-1 triggers a switch (SW) from  negative to positive regulation.	bind
10124	4	4039	5	11	NULL	NULL	NULL	SW	Process		is					switch	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_132_23_5225_s_383	16267094	(B) MSP binding to VAB-1 triggers a switch (SW) from  negative to positive regulation.	bind
44761	2	4039	5	11	NULL	NULL	NULL	negative regulation	Process		switches to					positive regulation	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_132_23_5225_s_383	16267094	(B) MSP binding to VAB-1 triggers a switch (SW) from  negative to positive regulation.	bind
12498	1	4039	7	11	NULL	NULL	NULL	MSP	GP		bind					VAB-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_132_23_5225_s_383	16267094	(B) MSP binding to VAB-1 triggers a switch (SW) from  negative to positive regulation.	bind
12499	2	4039	7	11	NULL	NULL	NULL	negative regulation	Process		switches to					positive regulation	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_132_23_5225_s_383	16267094	(B) MSP binding to VAB-1 triggers a switch (SW) from  negative to positive regulation.	bind
12500	3	4039	7	11	NULL	NULL	NULL	switch	Process		is					SW	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_132_23_5225_s_383	16267094	(B) MSP binding to VAB-1 triggers a switch (SW) from  negative to positive regulation.	bind
54247	4	4039	7	11	NULL	NULL	NULL	statement 1	Process		triggers					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_132_23_5225_s_383	16267094	(B) MSP binding to VAB-1 triggers a switch (SW) from  negative to positive regulation.	bind
10571	1	4040	5	11	NULL	NULL	NULL	MST1	GP		bind					NORE	GP		carboxy-terminal to RA domain		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_4_253_s_55	11864565	(B) MST1 binds NORE carboxy-terminal to the NORE-RA domain.	bind
18467	1	4040	7	11	NULL	NULL	NULL	MST1	GP		binds					NORE	GP		carboxy-terminal to the RA domain		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_4_253_s_55	11864565	(B) MST1 binds NORE carboxy-terminal to the NORE-RA domain.	bind
10125	1	4041	5	11	NULL	NULL	NULL	TBP	GP		bind					nhp6ab mot1 strain	GP		R1243I		NULL		NULL	NULL	NULL	NULL	gw70_genetics_172_2_837_s_242	16272410	(B) Multicopy TBP plasmid restores TBP binding in the   nhp6ab mot1(R1243I) strain.	bind
10126	2	4041	5	11	NULL	NULL	NULL	TBP plasmid	CellComponent	multicopy	restores					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_genetics_172_2_837_s_242	16272410	(B) Multicopy TBP plasmid restores TBP binding in the   nhp6ab mot1(R1243I) strain.	bind
12504	1	4041	7	11	NULL	NULL	NULL	TBP	GP		bind					nhp6ab mot1  strain	GP		R1243I		NULL		NULL	NULL	NULL	NULL	gw70_genetics_172_2_837_s_242	16272410	(B) Multicopy TBP plasmid restores TBP binding in the   nhp6ab mot1(R1243I) strain.	bind
15600	2	4041	7	11	NULL	NULL	NULL	TBP plasmid	GP	multicopy	restores					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_genetics_172_2_837_s_242	16272410	(B) Multicopy TBP plasmid restores TBP binding in the   nhp6ab mot1(R1243I) strain.	bind
10133	1	4043	5	11	NULL	NULL	NULL	ATP	Chemical		bind					ABC transporters	GP				NULL		NULL	NULL	NULL	NULL	gw60_genetics_152_4_1417_s_176	10430572	(B) Multiple sequence alignment of partial ORF1 with the five most similar database entries, all of which are ATP-binding subunits of ABC transporters.	bind
12507	1	4043	7	11	NULL	NULL	NULL	ATP	Chemical		bind					ABC transporter	GP				NULL		NULL	NULL	NULL	NULL	gw60_genetics_152_4_1417_s_176	10430572	(B) Multiple sequence alignment of partial ORF1 with the five most similar database entries, all of which are ATP-binding subunits of ABC transporters.	bind
10136	1	4044	5	11	NULL	NULL	NULL	RB proteins	GP	mutant	does not bind					E2F-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_5_1390_s_134	11839806	(B) Mutant RB proteins do not bind more E2F-1.	bind
12508	1	4044	7	11	NULL	NULL	NULL	RB protein	GP	mutant	does not bind					E2F-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_5_1390_s_134	11839806	(B) Mutant RB proteins do not bind more E2F-1.	bind
10579	1	4045	5	11	NULL	NULL	NULL	ZEBRA	GP		bind		cooperatively			HMG-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_190	10825199	(B) Mutation of individual ZEBRA binding sites abolishes cooperative binding of ZEBRA and HMG-1.	bind
10580	2	4045	5	11	NULL	NULL	NULL	ZEBRA	GP	mutant	abolish			binding sites		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_190	10825199	(B) Mutation of individual ZEBRA binding sites abolishes cooperative binding of ZEBRA and HMG-1.	bind
12509	1	4045	7	11	NULL	NULL	NULL	ZEBRA	GP		bind		cooperatively			HMG-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_190	10825199	(B) Mutation of individual ZEBRA binding sites abolishes cooperative binding of ZEBRA and HMG-1.	bind
12510	2	4045	7	11	NULL	NULL	NULL	ZEBRA	GP	mutant	abolishes			binding site		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_190	10825199	(B) Mutation of individual ZEBRA binding sites abolishes cooperative binding of ZEBRA and HMG-1.	bind
10141	1	4046	5	11	NULL	NULL	NULL	D-STAT	GP		undergoes							phosphorylation of	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_cell_84_3_421_s_104	8608596	(B) Mutation of Tyr-704  to Phe-704 abolished the tyrosine phosphorylation of D-STAT.	bind
10142	2	4046	5	11	NULL	NULL	NULL			mutation of	abolish			Tyr-704		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_84_3_421_s_104	8608596	(B) Mutation of Tyr-704  to Phe-704 abolished the tyrosine phosphorylation of D-STAT.	bind
10143	3	4046	5	11	NULL	NULL	NULL			mutation of	abolish			Phe-704		statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_84_3_421_s_104	8608596	(B) Mutation of Tyr-704  to Phe-704 abolished the tyrosine phosphorylation of D-STAT.	bind
12513	1	4046	7	11	NULL	NULL	NULL	D-STAT	GP		undergoes							phosphorylation of	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_cell_84_3_421_s_104	8608596	(B) Mutation of Tyr-704  to Phe-704 abolished the tyrosine phosphorylation of D-STAT.	bind
15601	2	4046	7	11	NULL	NULL	NULL			mutation	abolish			Tyr-704 		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_84_3_421_s_104	8608596	(B) Mutation of Tyr-704  to Phe-704 abolished the tyrosine phosphorylation of D-STAT.	bind
15602	3	4046	7	11	NULL	NULL	NULL			mutation	abolish			Phe-704		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_84_3_421_s_104	8608596	(B) Mutation of Tyr-704  to Phe-704 abolished the tyrosine phosphorylation of D-STAT.	bind
10144	1	4047	5	11	NULL	NULL	NULL	vIRF	GP		bind					p300	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_21_8254_s_120	11027294	(B) Mutational analysis of vIRF binding to p300.	bind
12514	1	4047	7	11	NULL	NULL	NULL	vIRF	GP		bind					p300	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_21_8254_s_120	11027294	(B) Mutational analysis of vIRF binding to p300.	bind
10148	1	4048	5	11	NULL	NULL	NULL	Arp2/3 complex	GP		mediate					actin	GP	nucleation of			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_89_s_70	11581288	(B) Mutations in the actin monomer-binding region of ActA decrease the efficiency of Arp2/3 complex -  mediated actin nucleation.	bind
10149	2	4048	5	11	NULL	NULL	NULL	ActA	GP	mutation in	decreases			actin monomer-binding region		statement 1	Process	efficieny of			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_89_s_70	11581288	(B) Mutations in the actin monomer-binding region of ActA decrease the efficiency of Arp2/3 complex -  mediated actin nucleation.	bind
12515	1	4048	7	11	NULL	NULL	NULL	Arp2/3 complex	GP		mediate					actin	GP	nucleation of			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_89_s_70	11581288	(B) Mutations in the actin monomer-binding region of ActA decrease the efficiency of Arp2/3 complex -  mediated actin nucleation.	bind
12516	2	4048	7	11	NULL	NULL	NULL	ActA	GP	mutations in	decrease			actin monomer-binding region		statement 1	Process	efficiency of			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_1_89_s_70	11581288	(B) Mutations in the actin monomer-binding region of ActA decrease the efficiency of Arp2/3 complex -  mediated actin nucleation.	bind
10581	1	4049	5	11	NULL	NULL	NULL	AMP	Chemical		bind					gamma2	GP		CBS domains		NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_113_2_274_s_178	14722619	(b) Mutations that caused an increase in the  B0.5 for binding of AMP to the CBS domains of gamma2 also caused an increase in the  A0.5 for activation of recombinant alpha1beta1gamma2 complexes, with the same order of potency, i.e.,  B0.5 or  A0.5 for WT   L ins < R302Q < H383R < T400N < R531G.	bind
12517	1	4049	7	11	NULL	NULL	NULL	AMP	Chemical		bind					gamma2	GP		CBS domain		NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_113_2_274_s_178	14722619	(b) Mutations that caused an increase in the  B0.5 for binding of AMP to the CBS domains of gamma2 also caused an increase in the  A0.5 for activation of recombinant alpha1beta1gamma2 complexes, with the same order of potency, i.e.,  B0.5 or  A0.5 for WT   L ins < R302Q < H383R < T400N < R531G.	bind
10150	1	4050	5	11	NULL	NULL	NULL	MutS/MutL	GP		bind									Sb-G/T-bS	NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_233_s_147	12887908	(B) MutS/MutL binding to biotin-streptavidin double blocked-end G/T mismatch DNA (Sb-G/T-bS).	bind
10151	2	4050	5	11	NULL	NULL	NULL	Sb-G/T-bS	NucleicAcid		is					biotin-streptavidin double blocked-end G/T mismatch DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_233_s_147	12887908	(B) MutS/MutL binding to biotin-streptavidin double blocked-end G/T mismatch DNA (Sb-G/T-bS).	bind
12518	1	4050	7	11	NULL	NULL	NULL	MutS/MutL	GP		bind									Sb-G/T-bS	NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_233_s_147	12887908	(B) MutS/MutL binding to biotin-streptavidin double blocked-end G/T mismatch DNA (Sb-G/T-bS).	bind
12519	2	4050	7	11	NULL	NULL	NULL	Sb-G/T-bS	NucleicAcid		is					biotin-streptavidin double blocked-end G/T mismatch DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_233_s_147	12887908	(B) MutS/MutL binding to biotin-streptavidin double blocked-end G/T mismatch DNA (Sb-G/T-bS).	bind
10152	1	4051	5	11	NULL	NULL	NULL	NFATp	GP		bind					TNF-alpha	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_8_2620_s_122	11909956	(B) Mutually exclusive binding of NFATp and Ets-1 to shared sites in the TNF-alpha promoter.	bind
10153	2	4051	5	11	NULL	NULL	NULL	Ets-1	GP		bind					TNF-alpha	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_8_2620_s_122	11909956	(B) Mutually exclusive binding of NFATp and Ets-1 to shared sites in the TNF-alpha promoter.	bind
10154	3	4051	5	11	NULL	NULL	NULL	statement 1	Process		mutually exclusive to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_8_2620_s_122	11909956	(B) Mutually exclusive binding of NFATp and Ets-1 to shared sites in the TNF-alpha promoter.	bind
12522	1	4051	7	11	NULL	NULL	NULL	NFATp	GP		bind					TNF-alpha	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_8_2620_s_122	11909956	(B) Mutually exclusive binding of NFATp and Ets-1 to shared sites in the TNF-alpha promoter.	bind
12524	2	4051	7	11	NULL	NULL	NULL	Ets-1	GP		bind					TNF-alpha	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_8_2620_s_122	11909956	(B) Mutually exclusive binding of NFATp and Ets-1 to shared sites in the TNF-alpha promoter.	bind
12526	3	4051	7	11	NULL	NULL	NULL	statement 1	Process		mutually exclusive to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_8_2620_s_122	11909956	(B) Mutually exclusive binding of NFATp and Ets-1 to shared sites in the TNF-alpha promoter.	bind
10155	1	4052	5	11	NULL	NULL	NULL	N-WASp	GP		bind					Arp2/3 complex	GP				NULL	at an actin filament branch point	NULL	NULL	NULL	NULL	gw60_currbiol_12_15_1270_s_226	12176354	(B) N-WASp and cortactin bound to Arp2/3 complex at an actin filament branch point.	bind
10156	2	4052	5	11	NULL	NULL	NULL	cortactin	GP		bind					Arp2/3 complex	GP				NULL	at an actin filament branch point	NULL	NULL	NULL	NULL	gw60_currbiol_12_15_1270_s_226	12176354	(B) N-WASp and cortactin bound to Arp2/3 complex at an actin filament branch point.	bind
12529	1	4052	7	11	NULL	NULL	NULL	N-WASp	GP		bind					Arp2/3 complex	GP				NULL	actin filament branch point	NULL	NULL	NULL	NULL	gw60_currbiol_12_15_1270_s_226	12176354	(B) N-WASp and cortactin bound to Arp2/3 complex at an actin filament branch point.	bind
12530	2	4052	7	11	NULL	NULL	NULL	cortactin	GP		bind					Arp2/3 complex	GP				NULL	actin filament branch point	NULL	NULL	NULL	NULL	gw60_currbiol_12_15_1270_s_226	12176354	(B) N-WASp and cortactin bound to Arp2/3 complex at an actin filament branch point.	bind
10157	1	4053	5	11	NULL	NULL	NULL	NBP1	GP		bind		tightly			Nef	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_8_5_647_s_45	9620685	(B) NBP1 binds to Nef tightly in the yeast two-hybrid system.	bind
12531	1	4053	7	11	NULL	NULL	NULL	NBP1	GP		bind		tightly			Nef	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_8_5_647_s_45	9620685	(B) NBP1 binds to Nef tightly in the yeast two-hybrid system.	bind
10158	1	4054	5	11	NULL	NULL	NULL	LDL	Chemical		bind		specifically			mSR-BI	GP				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_4_753_s_111	10191300	(B) Net specific binding activity of LDL to mSR-BI mediated by peptide V.	bind
10159	2	4054	5	11	NULL	NULL	NULL	statement 1	Process		is mediated by					peptide V	GP				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_4_753_s_111	10191300	(B) Net specific binding activity of LDL to mSR-BI mediated by peptide V.	bind
12532	1	4054	7	11	NULL	NULL	NULL	LDL	Chemical		bind		specifically			mSR-BI	GP				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_4_753_s_111	10191300	(B) Net specific binding activity of LDL to mSR-BI mediated by peptide V.	bind
12533	2	4054	7	11	NULL	NULL	NULL	statement 1	Process		is mediated by					peptide V	GP				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_4_753_s_111	10191300	(B) Net specific binding activity of LDL to mSR-BI mediated by peptide V.	bind
10160	1	4055	5	11	NULL	NULL	NULL	NeuAc4D ligand	Chemical		bind					BHA surface	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_structure_2_8_719_s_119	7994572	(b) NeuAc4D (carbon atoms colored yellow) ligand bound to the BHA surface.	bind
12534	1	4055	7	11	NULL	NULL	NULL	NeuAc4D	Chemical		bind					BHA surface	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_structure_2_8_719_s_119	7994572	(b) NeuAc4D (carbon atoms colored yellow) ligand bound to the BHA surface.	bind
10161	1	4058	5	11	NULL	NULL	NULL	NFI/CTF	GP		bind					CSF1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_cell_106_3_309_s_126	11509180	(B) NFI/CTF is bound to  CSF1 promoter in the absence of BAF  complex.	bind
10162	2	4058	5	11	NULL	NULL	NULL	statement 1	Process		in the absence of					BAF complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_106_3_309_s_126	11509180	(B) NFI/CTF is bound to  CSF1 promoter in the absence of BAF  complex.	bind
12535	1	4058	7	11	NULL	NULL	NULL	NFI/CTF	GP		bind					CSF1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_cell_106_3_309_s_126	11509180	(B) NFI/CTF is bound to  CSF1 promoter in the absence of BAF  complex.	bind
12536	2	4058	7	11	NULL	NULL	NULL	statement 1	Process		occurs in the absence of					BAF complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_106_3_309_s_126	11509180	(B) NFI/CTF is bound to  CSF1 promoter in the absence of BAF  complex.	bind
10163	1	4059	5	11	NULL	NULL	NULL	Nmd5p	GP		bind					Crz1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_951_s_112	11535618	(B) Nmd5p binds Crz1p in a calcineurin-dependent manner.	bind
10164	2	4059	5	11	NULL	NULL	NULL	statement 1	Process		is dependent on					calcineurin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_951_s_112	11535618	(B) Nmd5p binds Crz1p in a calcineurin-dependent manner.	bind
12537	1	4059	7	11	NULL	NULL	NULL	Nmd5p	GP		bind					Crz1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_951_s_112	11535618	(B) Nmd5p binds Crz1p in a calcineurin-dependent manner.	bind
12538	2	4059	7	11	NULL	NULL	NULL	statement 1	Process		is dependent on					calcineurin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_951_s_112	11535618	(B) Nmd5p binds Crz1p in a calcineurin-dependent manner.	bind
10165	1	4060	5	11	NULL	NULL	NULL	Npap60	GP		bind					importin-alpha:beta	GP				NULL	HeLa cytosol	NULL	NULL	NULL	NULL	gw60_cell_110_3_349_s_47	12176322	(B) Npap60 binds importin-alpha:beta from HeLa cytosol.	bind
12539	1	4060	7	11	NULL	NULL	NULL	Npap60	GP		binds					importin-alpha:beta	GP				NULL	HeLa cytosol	NULL	NULL	NULL	NULL	gw60_cell_110_3_349_s_47	12176322	(B) Npap60 binds importin-alpha:beta from HeLa cytosol.	bind
10166	1	4061	5	11	NULL	NULL	NULL	NSF	GP		bind					R2C-PICK1 complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_34_1_53_s_57	11931741	(B) NSF binds R2C-PICK1 complex more strongly than R2C alone.	bind
10167	2	4061	5	11	NULL	NULL	NULL	NSF	GP		bind					R2C	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_34_1_53_s_57	11931741	(B) NSF binds R2C-PICK1 complex more strongly than R2C alone.	bind
10168	3	4061	5	11	NULL	NULL	NULL	statement 1	Process		is stronger than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_34_1_53_s_57	11931741	(B) NSF binds R2C-PICK1 complex more strongly than R2C alone.	bind
12541	1	4061	7	11	NULL	NULL	NULL	NSF	GP		bind					R2C-PICK1 complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_34_1_53_s_57	11931741	(B) NSF binds R2C-PICK1 complex more strongly than R2C alone.	bind
12543	2	4061	7	11	NULL	NULL	NULL	NSF	GP		bind					R2C	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_34_1_53_s_57	11931741	(B) NSF binds R2C-PICK1 complex more strongly than R2C alone.	bind
12544	3	4061	7	11	NULL	NULL	NULL	statement 1	Process		occurs  more strongly than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_34_1_53_s_57	11931741	(B) NSF binds R2C-PICK1 complex more strongly than R2C alone.	bind
10169	1	4062	5	11	NULL	NULL	NULL	NTF2	GP		bind					Ran GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_5_1241_s_147	12769848	(B) NTF2 bound to Ran GDP.	bind
12546	1	4062	7	11	NULL	NULL	NULL	NTF2	GP		bind					Ran GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_5_1241_s_147	12769848	(B) NTF2 bound to Ran GDP.	bind
10170	1	4064	5	11	NULL	NULL	NULL	HMG-17	GP	heat-treated	bind					Cp	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3466_s_223	10207070	(B) Nucleoprotein gel assay showing that heat-treated (95 degrees C, 5 min) HMG-17 bound to core particles (Cp) in a manner that is indistinguishable from the untreated HMG-17.	bind
10171	2	4064	5	11	NULL	NULL	NULL	Cp	CellComponent		is					core particles	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3466_s_223	10207070	(B) Nucleoprotein gel assay showing that heat-treated (95 degrees C, 5 min) HMG-17 bound to core particles (Cp) in a manner that is indistinguishable from the untreated HMG-17.	bind
10172	3	4064	5	11	NULL	NULL	NULL	HMG-17	GP	untreated	bind					Cp	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3466_s_223	10207070	(B) Nucleoprotein gel assay showing that heat-treated (95 degrees C, 5 min) HMG-17 bound to core particles (Cp) in a manner that is indistinguishable from the untreated HMG-17.	bind
10173	4	4064	5	11	NULL	NULL	NULL	statement 1	Process		is indistinguishable from					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3466_s_223	10207070	(B) Nucleoprotein gel assay showing that heat-treated (95 degrees C, 5 min) HMG-17 bound to core particles (Cp) in a manner that is indistinguishable from the untreated HMG-17.	bind
12547	1	4064	7	11	NULL	NULL	NULL	HMG-17	GP	heat-treated	bind					Cp	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3466_s_223	10207070	(B) Nucleoprotein gel assay showing that heat-treated (95 degrees C, 5 min) HMG-17 bound to core particles (Cp) in a manner that is indistinguishable from the untreated HMG-17.	bind
12548	2	4064	7	11	NULL	NULL	NULL	Cp	CellComponent		is					core particles	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3466_s_223	10207070	(B) Nucleoprotein gel assay showing that heat-treated (95 degrees C, 5 min) HMG-17 bound to core particles (Cp) in a manner that is indistinguishable from the untreated HMG-17.	bind
15603	3	4064	7	11	NULL	NULL	NULL	HMG-17	GP	untreated	bind					Cp	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3466_s_223	10207070	(B) Nucleoprotein gel assay showing that heat-treated (95 degrees C, 5 min) HMG-17 bound to core particles (Cp) in a manner that is indistinguishable from the untreated HMG-17.	bind
15605	4	4064	7	11	NULL	NULL	NULL	statement 1	Process		is indistinguishable from					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3466_s_223	10207070	(B) Nucleoprotein gel assay showing that heat-treated (95 degrees C, 5 min) HMG-17 bound to core particles (Cp) in a manner that is indistinguishable from the untreated HMG-17.	bind
10174	1	4065	5	11	NULL	NULL	NULL	NXF	GP		bind		directly			Drebrin	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_2_608_s_94	14701734	(b) NXF directly binds to the Drebrin promoter in vivo.	bind
12554	1	4065	7	11	NULL	NULL	NULL	NXF	GP		bind		directly			Drebrin	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_2_608_s_94	14701734	(b) NXF directly binds to the Drebrin promoter in vivo.	bind
10175	1	4066	5	11	NULL	NULL	NULL	NXT1	GP		bind		directly			Crm1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_1_141_s_240	11149927	(B) NXT1 binds directly to Crm1, and binding is stimulated by the addition of Ran preloaded with GMP-PNP.	bind
10176	3	4066	5	11	NULL	NULL	NULL	statement 1	Process		is stimulated by					statement 2	Process	addition of			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_1_141_s_240	11149927	(B) NXT1 binds directly to Crm1, and binding is stimulated by the addition of Ran preloaded with GMP-PNP.	bind
10177	2	4066	5	11	NULL	NULL	NULL	Ran	GP		preloaded with					GMP-PNP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_1_141_s_240	11149927	(B) NXT1 binds directly to Crm1, and binding is stimulated by the addition of Ran preloaded with GMP-PNP.	bind
12555	1	4066	7	11	NULL	NULL	NULL	NXT1	GP		bind		directly			Crm1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_1_141_s_240	11149927	(B) NXT1 binds directly to Crm1, and binding is stimulated by the addition of Ran preloaded with GMP-PNP.	bind
12556	2	4066	7	11	NULL	NULL	NULL	Ran	GP		stimulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_1_141_s_240	11149927	(B) NXT1 binds directly to Crm1, and binding is stimulated by the addition of Ran preloaded with GMP-PNP.	bind
12558	3	4066	7	11	NULL	NULL	NULL	Ran	GP		is preloaded with					GMP-PNP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_1_141_s_240	11149927	(B) NXT1 binds directly to Crm1, and binding is stimulated by the addition of Ran preloaded with GMP-PNP.	bind
10178	1	4067	5	11	NULL	NULL	NULL	OAS1D	GP		bind					OAS1A	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_11_4615_s_262	15899864	(B) OAS1D binds OAS1A in vitro.	bind
12561	1	4067	7	11	NULL	NULL	NULL	OAS1D	GP		binds					OAS1A	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_11_4615_s_262	15899864	(B) OAS1D binds OAS1A in vitro.	bind
10179	1	4068	5	11	NULL	NULL	NULL	Sed5p	GP		bind		only			Sly1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_4_645_s_40	11994317	(B) Of the yeast ER to Golgi SNAREs, only Sed5p binds Sly1p.	bind
12563	1	4068	7	11	NULL	NULL	NULL	Sed5p	GP		binds					Sly1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_4_645_s_40	11994317	(B) Of the yeast ER to Golgi SNAREs, only Sed5p binds Sly1p.	bind
10180	1	4070	5	11	NULL	NULL	NULL	stimulus	Process		activate					Rac	GP				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_46_3_299_s_169	14975685	(B) Once a stimulus activates Rac, GTP bound Rac binds to Nap125,  PIR121 and Abi2, thus releasing WAVE1 and HSPC300.	bind
10181	2	4070	5	11	NULL	NULL	NULL	GTP	Chemical		bind					Rac	GP				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_46_3_299_s_169	14975685	(B) Once a stimulus activates Rac, GTP bound Rac binds to Nap125,  PIR121 and Abi2, thus releasing WAVE1 and HSPC300.	bind
10183	3	4070	5	11	NULL	NULL	NULL	statement 2	Process		bind					Nap125	GP				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_46_3_299_s_169	14975685	(B) Once a stimulus activates Rac, GTP bound Rac binds to Nap125,  PIR121 and Abi2, thus releasing WAVE1 and HSPC300.	bind
10184	4	4070	5	11	NULL	NULL	NULL	statement 2	Process		bind					PIR121	GP				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_46_3_299_s_169	14975685	(B) Once a stimulus activates Rac, GTP bound Rac binds to Nap125,  PIR121 and Abi2, thus releasing WAVE1 and HSPC300.	bind
10185	5	4070	5	11	NULL	NULL	NULL	statement 2	GP		bind					Abi2	GP				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_46_3_299_s_169	14975685	(B) Once a stimulus activates Rac, GTP bound Rac binds to Nap125,  PIR121 and Abi2, thus releasing WAVE1 and HSPC300.	bind
10186	6	4070	5	11	NULL	NULL	NULL	statement 3	Process		release					WAVE1	GP				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_46_3_299_s_169	14975685	(B) Once a stimulus activates Rac, GTP bound Rac binds to Nap125,  PIR121 and Abi2, thus releasing WAVE1 and HSPC300.	bind
10187	7	4070	5	11	NULL	NULL	NULL	statement 3	Process		release					HSPC300	GP				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_46_3_299_s_169	14975685	(B) Once a stimulus activates Rac, GTP bound Rac binds to Nap125,  PIR121 and Abi2, thus releasing WAVE1 and HSPC300.	bind
10188	8	4070	5	11	NULL	NULL	NULL	statement 4	Process		release					WAVE1	GP				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_46_3_299_s_169	14975685	(B) Once a stimulus activates Rac, GTP bound Rac binds to Nap125,  PIR121 and Abi2, thus releasing WAVE1 and HSPC300.	bind
10189	9	4070	5	11	NULL	NULL	NULL	statement 4	Process		release					HSPC300	GP				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_46_3_299_s_169	14975685	(B) Once a stimulus activates Rac, GTP bound Rac binds to Nap125,  PIR121 and Abi2, thus releasing WAVE1 and HSPC300.	bind
10190	10	4070	5	11	NULL	NULL	NULL	statement 5	Process		release					WAVE1	GP				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_46_3_299_s_169	14975685	(B) Once a stimulus activates Rac, GTP bound Rac binds to Nap125,  PIR121 and Abi2, thus releasing WAVE1 and HSPC300.	bind
10191	11	4070	5	11	NULL	NULL	NULL	statement 5	Process		release					HSPC300	GP				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_46_3_299_s_169	14975685	(B) Once a stimulus activates Rac, GTP bound Rac binds to Nap125,  PIR121 and Abi2, thus releasing WAVE1 and HSPC300.	bind
12564	1	4070	7	11	NULL	NULL	NULL	stimulus	Process		activates					Rac	GP				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_46_3_299_s_169	14975685	(B) Once a stimulus activates Rac, GTP bound Rac binds to Nap125,  PIR121 and Abi2, thus releasing WAVE1 and HSPC300.	bind
12565	3	4070	7	11	NULL	NULL	NULL	statement 2	Process		binds					Nap125	GP				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_46_3_299_s_169	14975685	(B) Once a stimulus activates Rac, GTP bound Rac binds to Nap125,  PIR121 and Abi2, thus releasing WAVE1 and HSPC300.	bind
12566	4	4070	7	11	NULL	NULL	NULL	statement 2	GP		binds					PIR121	GP				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_46_3_299_s_169	14975685	(B) Once a stimulus activates Rac, GTP bound Rac binds to Nap125,  PIR121 and Abi2, thus releasing WAVE1 and HSPC300.	bind
12567	5	4070	7	11	NULL	NULL	NULL	statement 2	GP		binds					Abi2	GP				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_46_3_299_s_169	14975685	(B) Once a stimulus activates Rac, GTP bound Rac binds to Nap125,  PIR121 and Abi2, thus releasing WAVE1 and HSPC300.	bind
12569	6	4070	7	11	NULL	NULL	NULL	statement 3	Process		release					WAVE1	GP				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_46_3_299_s_169	14975685	(B) Once a stimulus activates Rac, GTP bound Rac binds to Nap125,  PIR121 and Abi2, thus releasing WAVE1 and HSPC300.	bind
12572	7	4070	7	11	NULL	NULL	NULL	statement 4	Process		release					WAVE1	GP				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_46_3_299_s_169	14975685	(B) Once a stimulus activates Rac, GTP bound Rac binds to Nap125,  PIR121 and Abi2, thus releasing WAVE1 and HSPC300.	bind
12573	8	4070	7	11	NULL	NULL	NULL	statement 5	Process		release					WAVE1	GP				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_46_3_299_s_169	14975685	(B) Once a stimulus activates Rac, GTP bound Rac binds to Nap125,  PIR121 and Abi2, thus releasing WAVE1 and HSPC300.	bind
12574	9	4070	7	11	NULL	NULL	NULL	statement 3	Process		release					HSPC300	GP				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_46_3_299_s_169	14975685	(B) Once a stimulus activates Rac, GTP bound Rac binds to Nap125,  PIR121 and Abi2, thus releasing WAVE1 and HSPC300.	bind
12575	10	4070	7	11	NULL	NULL	NULL	statement 4	Process		release					HSPC300	GP				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_46_3_299_s_169	14975685	(B) Once a stimulus activates Rac, GTP bound Rac binds to Nap125,  PIR121 and Abi2, thus releasing WAVE1 and HSPC300.	bind
12577	11	4070	7	11	NULL	NULL	NULL	statement 5	Process		release					HSPC300	GP				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_46_3_299_s_169	14975685	(B) Once a stimulus activates Rac, GTP bound Rac binds to Nap125,  PIR121 and Abi2, thus releasing WAVE1 and HSPC300.	bind
44406	2	4070	7	11	NULL	NULL	NULL	Rac	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_46_3_299_s_169	14975685	(B) Once a stimulus activates Rac, GTP bound Rac binds to Nap125,  PIR121 and Abi2, thus releasing WAVE1 and HSPC300.	bind
10192	1	4071	5	11	NULL	NULL	NULL	STAT1	GP		bind					DMA antibodies	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_104_5_731_s_68	11257227	(B) Only  methylated STAT1(NH2)-GST competes for STAT1 binding to  DMA antibodies.	bind
10193	2	4071	5	11	NULL	NULL	NULL	STAT1-GST	GP	methylated	bind			NH2		DMA antibodies	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_104_5_731_s_68	11257227	(B) Only  methylated STAT1(NH2)-GST competes for STAT1 binding to  DMA antibodies.	bind
10194	3	4071	5	11	NULL	NULL	NULL	statement 2	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_104_5_731_s_68	11257227	(B) Only  methylated STAT1(NH2)-GST competes for STAT1 binding to  DMA antibodies.	bind
12578	1	4071	7	11	NULL	NULL	NULL	STAT1	GP		bind					DMA antibodies	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_104_5_731_s_68	11257227	(B) Only  methylated STAT1(NH2)-GST competes for STAT1 binding to  DMA antibodies.	bind
12579	2	4071	7	11	NULL	NULL	NULL	STAT1-GST	GP	methylated	bind			NH2		DMA antibodies	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_104_5_731_s_68	11257227	(B) Only  methylated STAT1(NH2)-GST competes for STAT1 binding to  DMA antibodies.	bind
12581	3	4071	7	11	NULL	NULL	NULL	statement 2	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_104_5_731_s_68	11257227	(B) Only  methylated STAT1(NH2)-GST competes for STAT1 binding to  DMA antibodies.	bind
10195	1	4072	5	11	NULL	NULL	NULL	p53	GP		bind					DNA	NucleicAcid	platinated			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1517_3_392_s_99	11342217	(B) p53 binding to platinated DNA.	bind
12600	1	4072	7	11	NULL	NULL	NULL	p53	GP		bind					 DNA	NucleicAcid	platinated			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1517_3_392_s_99	11342217	(B) p53 binding to platinated DNA.	bind
10196	1	4073	5	11	NULL	NULL	NULL	p70 MGR	GP		bind					Dopa decarboxylase	GP	Drosophila		promoter	NULL		NULL	NULL	NULL	NULL	gw60_mechdev_114_1_37_s_154	12175488	(B) p70 MGR binds to the  Drosophila Dopa decarboxylase promoter.	bind
12601	1	4073	7	11	NULL	NULL	NULL	p70 MGR	GP		binds					Dopa decarboxylase	GP	Drosophila		promoter	NULL		NULL	NULL	NULL	NULL	gw60_mechdev_114_1_37_s_154	12175488	(B) p70 MGR binds to the  Drosophila Dopa decarboxylase promoter.	bind
10197	1	4074	5	11	NULL	NULL	NULL	PAI-2	GP		bind					Rb	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6520_s_148	12944478	(B) PAI-2 binds Rb and p130 but not p107.	bind
10198	2	4074	5	11	NULL	NULL	NULL	PAI-2	GP		bind					p130	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6520_s_148	12944478	(B) PAI-2 binds Rb and p130 but not p107.	bind
10199	3	4074	5	11	NULL	NULL	NULL	PAI-2	GP		does not bind					p107	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6520_s_148	12944478	(B) PAI-2 binds Rb and p130 but not p107.	bind
12602	1	4074	7	11	NULL	NULL	NULL	PAI-2	GP		binds					Rb	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6520_s_148	12944478	(B) PAI-2 binds Rb and p130 but not p107.	bind
12603	2	4074	7	11	NULL	NULL	NULL	PAI-2	GP		binds					p130	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6520_s_148	12944478	(B) PAI-2 binds Rb and p130 but not p107.	bind
12606	3	4074	7	11	NULL	NULL	NULL	PAI-2	GP		does not bind					p107	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6520_s_148	12944478	(B) PAI-2 binds Rb and p130 but not p107.	bind
10200	1	4075	5	11	NULL	NULL	NULL	Pax4	GP		bind			PD		Pax6	GP	putative 	target sites		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8281_s_158	10567553	(B) Pax4 PD binds to the putative Pax6 target sites.	bind
12607	1	4075	7	11	NULL	NULL	NULL	Pax4 	GP		binds to			PD		Pax6	GP	putative	target site		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8281_s_158	10567553	(B) Pax4 PD binds to the putative Pax6 target sites.	bind
10201	1	4076	5	11	NULL	NULL	NULL	p53	GP		bind					CBP	GP		KIX domain		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4849_s_91	10848610	(B) pCREB, but not unphosphorylated CREB, enhances p53 binding to the KIX domain of CBP.	bind
10202	2	4076	5	11	NULL	NULL	NULL	pCREB	GP		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4849_s_91	10848610	(B) pCREB, but not unphosphorylated CREB, enhances p53 binding to the KIX domain of CBP.	bind
10203	3	4076	5	11	NULL	NULL	NULL	CREB	GP	unphosphorylated	does not enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4849_s_91	10848610	(B) pCREB, but not unphosphorylated CREB, enhances p53 binding to the KIX domain of CBP.	bind
12608	1	4076	7	11	NULL	NULL	NULL	p53	GP		bind					CBP	GP		KIX		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4849_s_91	10848610	(B) pCREB, but not unphosphorylated CREB, enhances p53 binding to the KIX domain of CBP.	bind
12609	2	4076	7	11	NULL	NULL	NULL	pCREB	GP		enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4849_s_91	10848610	(B) pCREB, but not unphosphorylated CREB, enhances p53 binding to the KIX domain of CBP.	bind
12610	3	4076	7	11	NULL	NULL	NULL	CREB	GP	unphosphorylated	does not enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4849_s_91	10848610	(B) pCREB, but not unphosphorylated CREB, enhances p53 binding to the KIX domain of CBP.	bind
11430	1	4077	5	11	NULL	NULL	NULL	PTP1B	GP		bind					IR peptides	GP	monophosphorylated			NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_6_1401_s_58	11163213	(B) Peptide competition assay with the PTP1B substrate-trapping mutant form (D181A) quantifying the relative binding affinity of PTP1B for the mono-, bis-, and trisphosphorylated IR peptides.	bind
11431	2	4077	5	11	NULL	NULL	NULL	PTP1B	GP		bind					IR peptides	GP	bisphosphorylated			NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_6_1401_s_58	11163213	(B) Peptide competition assay with the PTP1B substrate-trapping mutant form (D181A) quantifying the relative binding affinity of PTP1B for the mono-, bis-, and trisphosphorylated IR peptides.	bind
11432	3	4077	5	11	NULL	NULL	NULL	PTP1B	GP		bind					IR peptides	GP	trisphosphorylated			NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_6_1401_s_58	11163213	(B) Peptide competition assay with the PTP1B substrate-trapping mutant form (D181A) quantifying the relative binding affinity of PTP1B for the mono-, bis-, and trisphosphorylated IR peptides.	bind
12611	1	4077	7	11	NULL	NULL	NULL	PTP1B	GP		bind					IR peptides	GP	monophosphorylated			NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_6_1401_s_58	11163213	(B) Peptide competition assay with the PTP1B substrate-trapping mutant form (D181A) quantifying the relative binding affinity of PTP1B for the mono-, bis-, and trisphosphorylated IR peptides.	bind
12612	2	4077	7	11	NULL	NULL	NULL	PTP1B	GP		bind					IR peptides	GP	bisphosphorylated			NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_6_1401_s_58	11163213	(B) Peptide competition assay with the PTP1B substrate-trapping mutant form (D181A) quantifying the relative binding affinity of PTP1B for the mono-, bis-, and trisphosphorylated IR peptides.	bind
12613	3	4077	7	11	NULL	NULL	NULL	PTP1B	GP		bind					IR peptides	GP	trisphosphorylated			NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_6_1401_s_58	11163213	(B) Peptide competition assay with the PTP1B substrate-trapping mutant form (D181A) quantifying the relative binding affinity of PTP1B for the mono-, bis-, and trisphosphorylated IR peptides.	bind
10204	1	4078	5	11	NULL	NULL	NULL	[3]BPTI	GP	unfolded	bind					EF-Tu	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_3_749_s_30	12176046	(B) Peptides  (DnaK binder) and  (not DnaK binder) were tested for their abillity to compete in solution for the binding of unfolded [3]BPTI to EF-Tu by gel permeation chromatography.	bind
12638	1	4078	7	11	NULL	NULL	NULL	[3]BPTI 	GP	unfolded	bind					EF-Tu	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_3_749_s_30	12176046	(B) Peptides  (DnaK binder) and  (not DnaK binder) were tested for their abillity to compete in solution for the binding of unfolded [3]BPTI to EF-Tu by gel permeation chromatography.	bind
10205	1	4079	5	11	NULL	NULL	NULL	MBL	GP		bind					bacteria	Organism				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_2_1052_s_206	15664949	(B) Percentages of MBL, L-ficolin, and H-ficolin bound to bacteria.	bind
10206	2	4079	5	11	NULL	NULL	NULL	L-ficolin	GP		bind					bacteria	Organism				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_2_1052_s_206	15664949	(B) Percentages of MBL, L-ficolin, and H-ficolin bound to bacteria.	bind
10207	3	4079	5	11	NULL	NULL	NULL	H-ficolin	GP		bind					bacteria	Organism				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_2_1052_s_206	15664949	(B) Percentages of MBL, L-ficolin, and H-ficolin bound to bacteria.	bind
12639	1	4079	7	11	NULL	NULL	NULL	MBL	GP		bind					bacteria	Organism				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_2_1052_s_206	15664949	(B) Percentages of MBL, L-ficolin, and H-ficolin bound to bacteria.	bind
12640	2	4079	7	11	NULL	NULL	NULL	L-ficolin	GP		bind					bacteria	Organism				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_2_1052_s_206	15664949	(B) Percentages of MBL, L-ficolin, and H-ficolin bound to bacteria.	bind
12641	3	4079	7	11	NULL	NULL	NULL	H-ficolin	GP		bind					bacteria	Organism				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_2_1052_s_206	15664949	(B) Percentages of MBL, L-ficolin, and H-ficolin bound to bacteria.	bind
10208	1	4082	5	11	NULL	NULL	NULL	Pex22p	GP		bind					Pex4p	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_cellbiol_146_1_99_s_311	10402463	(B) Pex22p binds to Pex4p in vivo.	bind
12642	1	4082	7	11	NULL	NULL	NULL	Pex22p	GP		binds to					Pex4p	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_cellbiol_146_1_99_s_311	10402463	(B) Pex22p binds to Pex4p in vivo.	bind
10209	1	4083	5	11	NULL	NULL	NULL	Mot1p	GP		bind					HXT	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_4863_s_201	15923605	(B) PhosphorImager quantification of Mot1p, Taf1p, TBP, and Pol II binding to the  indicated  HXT promoters.	bind
10210	2	4083	5	11	NULL	NULL	NULL	Taf1p	GP		bind					HXT	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_4863_s_201	15923605	(B) PhosphorImager quantification of Mot1p, Taf1p, TBP, and Pol II binding to the  indicated  HXT promoters.	bind
10211	3	4083	5	11	NULL	NULL	NULL	TBP	GP		bind					HXT	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_4863_s_201	15923605	(B) PhosphorImager quantification of Mot1p, Taf1p, TBP, and Pol II binding to the  indicated  HXT promoters.	bind
10212	4	4083	5	11	NULL	NULL	NULL	Pol II	GP		bind					HXT	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_4863_s_201	15923605	(B) PhosphorImager quantification of Mot1p, Taf1p, TBP, and Pol II binding to the  indicated  HXT promoters.	bind
12643	1	4083	7	11	NULL	NULL	NULL	Mot1p	GP		bind					HXT	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_4863_s_201	15923605	(B) PhosphorImager quantification of Mot1p, Taf1p, TBP, and Pol II binding to the  indicated  HXT promoters.	bind
12644	2	4083	7	11	NULL	NULL	NULL	Taf1p	GP		bind					HXT	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_4863_s_201	15923605	(B) PhosphorImager quantification of Mot1p, Taf1p, TBP, and Pol II binding to the  indicated  HXT promoters.	bind
12645	3	4083	7	11	NULL	NULL	NULL	TBP	GP		bind					HXT	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_4863_s_201	15923605	(B) PhosphorImager quantification of Mot1p, Taf1p, TBP, and Pol II binding to the  indicated  HXT promoters.	bind
12646	4	4083	7	11	NULL	NULL	NULL	Pol II	GP		bind					HXT	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_4863_s_201	15923605	(B) PhosphorImager quantification of Mot1p, Taf1p, TBP, and Pol II binding to the  indicated  HXT promoters.	bind
10213	1	4085	5	11	NULL	NULL	NULL	AP-1	GP		bind					Golgi	CellComponent	semi-intact cells			NULL		NULL	NULL	NULL	NULL	gw60_cell_114_3_299_s_167	12914695	(B) PI(4)P addback restores AP-1 binding to the Golgi of semi-intact cells.	bind
10214	2	4085	5	11	NULL	NULL	NULL	PI(4)P	Chemical		restores					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_3_299_s_167	12914695	(B) PI(4)P addback restores AP-1 binding to the Golgi of semi-intact cells.	bind
12647	1	4085	7	11	NULL	NULL	NULL	AP-1	GP		bind					Golgi 	CellComponent	semi-intact cells			NULL		NULL	NULL	NULL	NULL	gw60_cell_114_3_299_s_167	12914695	(B) PI(4)P addback restores AP-1 binding to the Golgi of semi-intact cells.	bind
12648	2	4085	7	11	NULL	NULL	NULL	PI(4)P	Chemical		restores					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_3_299_s_167	12914695	(B) PI(4)P addback restores AP-1 binding to the Golgi of semi-intact cells.	bind
10215	1	4086	5	11	NULL	NULL	NULL	PlexB	GP		bind					Rac	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_1_39_s_57	11604137	(B) PlexB binds to Rac in a GTP-dependent manner.	bind
10216	2	4086	5	11	NULL	NULL	NULL	statement 1	Process		is dependent on					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_1_39_s_57	11604137	(B) PlexB binds to Rac in a GTP-dependent manner.	bind
12649	1	4086	7	11	NULL	NULL	NULL	PlexB	GP		bind					Rac 	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_1_39_s_57	11604137	(B) PlexB binds to Rac in a GTP-dependent manner.	bind
12650	2	4086	7	11	NULL	NULL	NULL	statement 1	Process		is dependent on					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_1_39_s_57	11604137	(B) PlexB binds to Rac in a GTP-dependent manner.	bind
10217	1	4088	5	11	NULL	NULL	NULL	TRAF6	GP		mediate					IKK	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_cell_103_2_351_s_131	11057907	(B) Point mutation at Cys-87 of  Ubc13 abolishes its ability to support TRAF6-mediated IKK activation.	bind
10218	2	4088	5	11	NULL	NULL	NULL	Ubc13	GP	point mutation	abolish			Cys-87		statement 1	Process	ability to support			NULL		NULL	NULL	NULL	NULL	gw60_cell_103_2_351_s_131	11057907	(B) Point mutation at Cys-87 of  Ubc13 abolishes its ability to support TRAF6-mediated IKK activation.	bind
12651	1	4088	7	11	NULL	NULL	NULL	TRAF6	GP		mediates					IKK	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_cell_103_2_351_s_131	11057907	(B) Point mutation at Cys-87 of  Ubc13 abolishes its ability to support TRAF6-mediated IKK activation.	bind
12652	2	4088	7	11	NULL	NULL	NULL	Ubc13	GP	Point mutation at	abolishes			Cys-87		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_2_351_s_131	11057907	(B) Point mutation at Cys-87 of  Ubc13 abolishes its ability to support TRAF6-mediated IKK activation.	bind
10219	1	4089	5	11	NULL	NULL	NULL	Poly(ADP-ribose)	Chemical		bind					hTRF2	GP	purified;;recombinant			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_4_1595_s_237	14749375	(B) Poly(ADP-ribose) binds to purified recombinant hTRF2.	bind
12653	1	4089	7	11	NULL	NULL	NULL	Poly ADP-ribose	Chemical		binds					 hTRF2	GP	purified			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_4_1595_s_237	14749375	(B) Poly(ADP-ribose) binds to purified recombinant hTRF2.	bind
10220	1	4090	5	11	NULL	NULL	NULL	p53	GP		bind		rapidly			mdm2	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_472_1_93_s_153	10781812	(B) Poly-G (5  g) precaptured by mdm2 bound to mAb 4B2 linked to the surface of a CM5 Biosensor chip, enhanced the binding of all the p53 mutations apart from p53C 64, showing that a tetramerisation domain is an absolute requirement for rapid binding of p53 to mdm2.	bind
10221	2	4090	5	11	NULL	NULL	NULL	mdm2	GP		bind					mAb 4B2	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_472_1_93_s_153	10781812	(B) Poly-G (5  g) precaptured by mdm2 bound to mAb 4B2 linked to the surface of a CM5 Biosensor chip, enhanced the binding of all the p53 mutations apart from p53C 64, showing that a tetramerisation domain is an absolute requirement for rapid binding of p53 to mdm2.	bind
10222	3	4090	5	11	NULL	NULL	NULL	Poly-G	NucleicAcid		precaptured by					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_472_1_93_s_153	10781812	(B) Poly-G (5  g) precaptured by mdm2 bound to mAb 4B2 linked to the surface of a CM5 Biosensor chip, enhanced the binding of all the p53 mutations apart from p53C 64, showing that a tetramerisation domain is an absolute requirement for rapid binding of p53 to mdm2.	bind
10223	4	4090	5	11	NULL	NULL	NULL	statement 3	Process		enhances					p53	GP	binding of;; mutant			NULL		NULL	NULL	NULL	NULL	gw60_febslett_472_1_93_s_153	10781812	(B) Poly-G (5  g) precaptured by mdm2 bound to mAb 4B2 linked to the surface of a CM5 Biosensor chip, enhanced the binding of all the p53 mutations apart from p53C 64, showing that a tetramerisation domain is an absolute requirement for rapid binding of p53 to mdm2.	bind
10224	5	4090	5	11	NULL	NULL	NULL	statement 3	Process		does not enhance					p53	GP	binding of;; mutant	C 64		NULL		NULL	NULL	NULL	NULL	gw60_febslett_472_1_93_s_153	10781812	(B) Poly-G (5  g) precaptured by mdm2 bound to mAb 4B2 linked to the surface of a CM5 Biosensor chip, enhanced the binding of all the p53 mutations apart from p53C 64, showing that a tetramerisation domain is an absolute requirement for rapid binding of p53 to mdm2.	bind
10225	6	4090	5	11	NULL	NULL	NULL				is required for		absolutely	tetramerisation domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_472_1_93_s_153	10781812	(B) Poly-G (5  g) precaptured by mdm2 bound to mAb 4B2 linked to the surface of a CM5 Biosensor chip, enhanced the binding of all the p53 mutations apart from p53C 64, showing that a tetramerisation domain is an absolute requirement for rapid binding of p53 to mdm2.	bind
10226	7	4090	5	11	NULL	NULL	NULL	statement 4	Process		shows					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_472_1_93_s_153	10781812	(B) Poly-G (5  g) precaptured by mdm2 bound to mAb 4B2 linked to the surface of a CM5 Biosensor chip, enhanced the binding of all the p53 mutations apart from p53C 64, showing that a tetramerisation domain is an absolute requirement for rapid binding of p53 to mdm2.	bind
10227	8	4090	5	11	NULL	NULL	NULL	statement 5	Process		shows					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_472_1_93_s_153	10781812	(B) Poly-G (5  g) precaptured by mdm2 bound to mAb 4B2 linked to the surface of a CM5 Biosensor chip, enhanced the binding of all the p53 mutations apart from p53C 64, showing that a tetramerisation domain is an absolute requirement for rapid binding of p53 to mdm2.	bind
12654	1	4090	7	11	NULL	NULL	NULL	Poly-G	NucleicAcid		bind					mAb 4B2	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_472_1_93_s_153	10781812	(B) Poly-G (5  g) precaptured by mdm2 bound to mAb 4B2 linked to the surface of a CM5 Biosensor chip, enhanced the binding of all the p53 mutations apart from p53C 64, showing that a tetramerisation domain is an absolute requirement for rapid binding of p53 to mdm2.	bind
12655	2	4090	7	11	NULL	NULL	NULL	Poly-G	NucleicAcid		is precaptured by					mdm2	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_472_1_93_s_153	10781812	(B) Poly-G (5  g) precaptured by mdm2 bound to mAb 4B2 linked to the surface of a CM5 Biosensor chip, enhanced the binding of all the p53 mutations apart from p53C 64, showing that a tetramerisation domain is an absolute requirement for rapid binding of p53 to mdm2.	bind
12661	5	4090	7	11	NULL	NULL	NULL	p53	GP		bind		rapidly			mdm2	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_472_1_93_s_153	10781812	(B) Poly-G (5  g) precaptured by mdm2 bound to mAb 4B2 linked to the surface of a CM5 Biosensor chip, enhanced the binding of all the p53 mutations apart from p53C 64, showing that a tetramerisation domain is an absolute requirement for rapid binding of p53 to mdm2.	bind
12664	6	4090	7	11	NULL	NULL	NULL				is required for			tetramerisation domain		statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_472_1_93_s_153	10781812	(B) Poly-G (5  g) precaptured by mdm2 bound to mAb 4B2 linked to the surface of a CM5 Biosensor chip, enhanced the binding of all the p53 mutations apart from p53C 64, showing that a tetramerisation domain is an absolute requirement for rapid binding of p53 to mdm2.	bind
44471	3	4090	7	11	NULL	NULL	NULL	statement 1	Process		enhance					p53	GP	binding of;;mutated			NULL		NULL	NULL	NULL	NULL	gw60_febslett_472_1_93_s_153	10781812	(B) Poly-G (5  g) precaptured by mdm2 bound to mAb 4B2 linked to the surface of a CM5 Biosensor chip, enhanced the binding of all the p53 mutations apart from p53C 64, showing that a tetramerisation domain is an absolute requirement for rapid binding of p53 to mdm2.	bind
44472	4	4090	7	11	NULL	NULL	NULL	statement 1	Process		does not enhance					p53	GP	binding of;;mutated	C64		NULL		NULL	NULL	NULL	NULL	gw60_febslett_472_1_93_s_153	10781812	(B) Poly-G (5  g) precaptured by mdm2 bound to mAb 4B2 linked to the surface of a CM5 Biosensor chip, enhanced the binding of all the p53 mutations apart from p53C 64, showing that a tetramerisation domain is an absolute requirement for rapid binding of p53 to mdm2.	bind
10228	1	4092	5	11	NULL	NULL	NULL	GST-Rad24	GP		bind		preferentially			phospho-Ste11	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_1_3_389_s_207	11702950	(B) Preferential binding between GST-Rad24 and phospho-Ste11.	bind
12665	1	4092	7	11	NULL	NULL	NULL	GST-Rad24	GP		bind		preferentially			phospho-Ste11	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_1_3_389_s_207	11702950	(B) Preferential binding between GST-Rad24 and phospho-Ste11.	bind
10229	1	4093	5	11	NULL	NULL	NULL	AF-6	GP		bind					Ras	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_13_4663_s_272	12808105	(B) Prevention of phosphorylation of AF-6 by  Bcr reduces binding of AF-6 to Ras.	bind
10230	2	4093	5	11	NULL	NULL	NULL	Bcr	GP		prevent					AF-6	GP	phosphorylation of 			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_13_4663_s_272	12808105	(B) Prevention of phosphorylation of AF-6 by  Bcr reduces binding of AF-6 to Ras.	bind
10231	3	4093	5	11	NULL	NULL	NULL	statement 2	Process		reduce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_13_4663_s_272	12808105	(B) Prevention of phosphorylation of AF-6 by  Bcr reduces binding of AF-6 to Ras.	bind
12666	1	4093	7	11	NULL	NULL	NULL	AF-6	GP		bind					Ras	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_13_4663_s_272	12808105	(B) Prevention of phosphorylation of AF-6 by  Bcr reduces binding of AF-6 to Ras.	bind
12667	2	4093	7	11	NULL	NULL	NULL	Bcr	GP		prevents					AF6	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_13_4663_s_272	12808105	(B) Prevention of phosphorylation of AF-6 by  Bcr reduces binding of AF-6 to Ras.	bind
12668	3	4093	7	11	NULL	NULL	NULL	statement 2	Process		reduce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_13_4663_s_272	12808105	(B) Prevention of phosphorylation of AF-6 by  Bcr reduces binding of AF-6 to Ras.	bind
10232	1	4096	5	11	NULL	NULL	NULL	Apaf1	GP		bind				promoter	p53	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_2_207_s_91	11591730	(B) Protein was extracted from neurons 48 h after infection with Ad-p53 or Ad-p53-173L and p53 binding activity to the Apaf1 promoter elements was assayed by electrophoretic mobility shift assay.	bind
12669	1	4096	7	11	NULL	NULL	NULL	 p53	GP		bind					Apaf1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_2_207_s_91	11591730	(B) Protein was extracted from neurons 48 h after infection with Ad-p53 or Ad-p53-173L and p53 binding activity to the Apaf1 promoter elements was assayed by electrophoretic mobility shift assay.	bind
10233	1	4097	5	11	NULL	NULL	NULL	c-Src	GP		phosphorylate					GST-PECAM	GP		1Cyt		NULL		NULL	NULL	NULL	NULL	gw60_febslett_408_3_331_s_73	9188788	(B) Proteins bound to the c-Src phosphorylated GST-PECAM-1Cyt affinity matrix.	bind
12670	1	4097	7	11	NULL	NULL	NULL	c-Src	GP		phosphorylate					GST-PECAM	GP		1Cyt		NULL		NULL	NULL	NULL	NULL	gw60_febslett_408_3_331_s_73	9188788	(B) Proteins bound to the c-Src phosphorylated GST-PECAM-1Cyt affinity matrix.	bind
10234	1	4104	5	11	NULL	NULL	NULL	Tra2	GP	purified	bind					RNA	NucleicAcid			A element	NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1625_2_141_s_196	12531473	(B) Purified Tra2  binds to A element RNA.	bind
12671	1	4104	7	11	NULL	NULL	NULL	Tra2 	GP	purified	bind					RNA	NucleicAcid			A element	NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1625_2_141_s_196	12531473	(B) Purified Tra2  binds to A element RNA.	bind
10235	1	4105	5	11	NULL	NULL	NULL	TWD1-3 protein	GP	purified	bind		specifically			vacuolar membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_7_3393_s_255	15133126	(B) Purified TWD1-3 protein binds specifically to vacuolar membranes.	bind
12672	1	4105	7	11	NULL	NULL	NULL	TWD1-3 	GP	purified	binds		specifically			vacuolar membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_7_3393_s_255	15133126	(B) Purified TWD1-3 protein binds specifically to vacuolar membranes.	bind
10236	1	4106	5	11	NULL	NULL	NULL	Ena 	GP	purified;;recombinant	bind					GST-Dlar	GP		D1-D2		NULL		NULL	NULL	NULL	NULL	gw60_neuron_22_2_301_s_196	10069336	(B) Purified, recombinant Ena (arrow) binds to GST-Dlar D1-D2 (lane 2), and binds weakly to GST-DPTP10D (lane 3) but does not bind significantly to GST alone (lane 1).	bind
10237	2	4106	5	11	NULL	NULL	NULL	Ena	GP	purified;;recombinant	bind		weakly			GST-DPTP10D	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_22_2_301_s_196	10069336	(B) Purified, recombinant Ena (arrow) binds to GST-Dlar D1-D2 (lane 2), and binds weakly to GST-DPTP10D (lane 3) but does not bind significantly to GST alone (lane 1).	bind
10238	3	4106	5	11	NULL	NULL	NULL	Ena	GP	purified;;recombinant	does not bind		significantly			GST	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_22_2_301_s_196	10069336	(B) Purified, recombinant Ena (arrow) binds to GST-Dlar D1-D2 (lane 2), and binds weakly to GST-DPTP10D (lane 3) but does not bind significantly to GST alone (lane 1).	bind
44473	1	4106	7	11	NULL	NULL	NULL	Ena	GP	purified;;recombinant	bind					GST-Dlar 	GP		D1-D2		NULL		NULL	NULL	NULL	NULL	gw60_neuron_22_2_301_s_196	10069336	(B) Purified, recombinant Ena (arrow) binds to GST-Dlar D1-D2 (lane 2), and binds weakly to GST-DPTP10D (lane 3) but does not bind significantly to GST alone (lane 1).	bind
44474	2	4106	7	11	NULL	NULL	NULL	Ena	GP	purified;;recombinant	bind		weakly			GST-DPTP10D	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_22_2_301_s_196	10069336	(B) Purified, recombinant Ena (arrow) binds to GST-Dlar D1-D2 (lane 2), and binds weakly to GST-DPTP10D (lane 3) but does not bind significantly to GST alone (lane 1).	bind
44476	3	4106	7	11	NULL	NULL	NULL	Ena	GP	purified;;recombinant	does not bind		significantly			GST	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_22_2_301_s_196	10069336	(B) Purified, recombinant Ena (arrow) binds to GST-Dlar D1-D2 (lane 2), and binds weakly to GST-DPTP10D (lane 3) but does not bind significantly to GST alone (lane 1).	bind
10239	1	4107	5	11	NULL	NULL	NULL	mSin3A	GP		bind									5' LTR	NULL	SLB-1 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_14_6117_s_190	15226416	(B) Quantification of mSin3A and  NCoR binding at the 5' and 3'' LTRs in SLB-1 cells.	bind
10240	2	4107	5	11	NULL	NULL	NULL	mSin3A	GP		bind									3'' LTR	NULL	SLB-1 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_14_6117_s_190	15226416	(B) Quantification of mSin3A and  NCoR binding at the 5' and 3'' LTRs in SLB-1 cells.	bind
10241	3	4107	5	11	NULL	NULL	NULL	NCoR	GP		bind									5' LTR	NULL	SLB-1 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_14_6117_s_190	15226416	(B) Quantification of mSin3A and  NCoR binding at the 5' and 3'' LTRs in SLB-1 cells.	bind
10242	4	4107	5	11	NULL	NULL	NULL	NCoR	GP		bind									3'' LTR	NULL	SLB-1 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_14_6117_s_190	15226416	(B) Quantification of mSin3A and  NCoR binding at the 5' and 3'' LTRs in SLB-1 cells.	bind
12677	1	4107	7	11	NULL	NULL	NULL	mSin3A	GP		bind									 5' LTR	NULL	SLB-1 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_14_6117_s_190	15226416	(B) Quantification of mSin3A and  NCoR binding at the 5' and 3'' LTRs in SLB-1 cells.	bind
12678	2	4107	7	11	NULL	NULL	NULL	mSin3A	GP		bind									3'' LTR	NULL	SLB-1 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_14_6117_s_190	15226416	(B) Quantification of mSin3A and  NCoR binding at the 5' and 3'' LTRs in SLB-1 cells.	bind
12680	4	4107	7	11	NULL	NULL	NULL	NCoR	GP		bind									3'' LTR	NULL	SLB-1 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_14_6117_s_190	15226416	(B) Quantification of mSin3A and  NCoR binding at the 5' and 3'' LTRs in SLB-1 cells.	bind
10243	1	4108	5	11	NULL	NULL	NULL	NodD1	GP		bind					nodF	GP		nod box		NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_15_5417_s_169	16855231	(B) Quantitation  of NodD1 binding to the  nodF nod box from the experiment shown in panel A.	bind
12679	3	4108	7	11	NULL	NULL	NULL	NCoR	GP		bind									5' LTR	NULL	SLB-1 cells	NULL	NULL	NULL	NULL	gw70_jbacteriol_188_15_5417_s_169	16855231	(B) Quantitation  of NodD1 binding to the  nodF nod box from the experiment shown in panel A.	bind
12681	1	4108	7	11	NULL	NULL	NULL	NodD1	GP		bind					nodF	GP		nod box		NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_15_5417_s_169	16855231	(B) Quantitation  of NodD1 binding to the  nodF nod box from the experiment shown in panel A.	bind
10244	1	4109	5	11	NULL	NULL	NULL	Spt10	GP		bind					HTA2-HTB2	GP			promoter	NULL	G1 phase	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_1_135_s_161	14673149	(B) Quantitation of Spt10  and Spt21 binding at the  HTA2-HTB2 promoter at both G1 (white bars) and S (gray bars) phases.	bind
10245	2	4109	5	11	NULL	NULL	NULL	Spt10	GP		bind					HTA2-HTB2	GP			promoter	NULL	S phase	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_1_135_s_161	14673149	(B) Quantitation of Spt10  and Spt21 binding at the  HTA2-HTB2 promoter at both G1 (white bars) and S (gray bars) phases.	bind
10246	3	4109	5	11	NULL	NULL	NULL	Spt21	GP		bind					HTA2-HTB2	GP			promoter	NULL	G1 phase	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_1_135_s_161	14673149	(B) Quantitation of Spt10  and Spt21 binding at the  HTA2-HTB2 promoter at both G1 (white bars) and S (gray bars) phases.	bind
10247	4	4109	5	11	NULL	NULL	NULL	Spt21	GP		bind					HTA2-HTB2	GP			promoter	NULL	S phase	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_1_135_s_161	14673149	(B) Quantitation of Spt10  and Spt21 binding at the  HTA2-HTB2 promoter at both G1 (white bars) and S (gray bars) phases.	bind
12682	1	4109	7	11	NULL	NULL	NULL	Spt10	GP		bind					HTA2-HTB2	GP			promoter	NULL	G1 phase	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_1_135_s_161	14673149	(B) Quantitation of Spt10  and Spt21 binding at the  HTA2-HTB2 promoter at both G1 (white bars) and S (gray bars) phases.	bind
12683	2	4109	7	11	NULL	NULL	NULL	Spt10	GP		bind					HTA2-HTB2	GP			promoter	NULL	S phase	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_1_135_s_161	14673149	(B) Quantitation of Spt10  and Spt21 binding at the  HTA2-HTB2 promoter at both G1 (white bars) and S (gray bars) phases.	bind
12684	3	4109	7	11	NULL	NULL	NULL	Spt21	GP		bind					HTA2-HTB2	GP			promoter	NULL	G1 phase	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_1_135_s_161	14673149	(B) Quantitation of Spt10  and Spt21 binding at the  HTA2-HTB2 promoter at both G1 (white bars) and S (gray bars) phases.	bind
12685	4	4109	7	11	NULL	NULL	NULL	Spt21	GP		bind					HTA2-HTB2	GP			promoter	NULL	S phase	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_1_135_s_161	14673149	(B) Quantitation of Spt10  and Spt21 binding at the  HTA2-HTB2 promoter at both G1 (white bars) and S (gray bars) phases.	bind
10248	1	4110	5	11	NULL	NULL	NULL	Pitx2 proteins 	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_7001_s_115	10490637	(B) Quantitation of the DNA binding of Pitx2 and truncated Pitx2 proteins from the EMSA experiments.	bind
10249	2	4110	5	11	NULL	NULL	NULL	Pitx2 proteins	GP	truncated	bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_7001_s_115	10490637	(B) Quantitation of the DNA binding of Pitx2 and truncated Pitx2 proteins from the EMSA experiments.	bind
12686	1	4110	7	11	NULL	NULL	NULL	Pitx2	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_7001_s_115	10490637	(B) Quantitation of the DNA binding of Pitx2 and truncated Pitx2 proteins from the EMSA experiments.	bind
12687	2	4110	7	11	NULL	NULL	NULL	Pitx2	GP	truncated	bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_7001_s_115	10490637	(B) Quantitation of the DNA binding of Pitx2 and truncated Pitx2 proteins from the EMSA experiments.	bind
10250	1	4111	5	11	NULL	NULL	NULL	acetyl-histone H3	GP		bind					bcl-2	GP			P1 promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1608_s_204	15713621	(B) Quantitative  ChIP assay of acetyl-histone H3 and acetyl-histone H4 binding to the  bcl-2 P1 promoter.	bind
10251	2	4111	5	11	NULL	NULL	NULL	acetyl-histone H4	GP		bind					bcl-2	GP			P1 promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1608_s_204	15713621	(B) Quantitative  ChIP assay of acetyl-histone H3 and acetyl-histone H4 binding to the  bcl-2 P1 promoter.	bind
12701	1	4111	7	11	NULL	NULL	NULL	acetyl-histone H3	GP		bind					bcl-2	GP			P1 promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1608_s_204	15713621	(B) Quantitative  ChIP assay of acetyl-histone H3 and acetyl-histone H4 binding to the  bcl-2 P1 promoter.	bind
12702	2	4111	7	11	NULL	NULL	NULL	acetyl-histone H4	GP		bind					bcl-2 	GP			P1 promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1608_s_204	15713621	(B) Quantitative  ChIP assay of acetyl-histone H3 and acetyl-histone H4 binding to the  bcl-2 P1 promoter.	bind
10252	1	4112	5	11	NULL	NULL	NULL	tubulin	GP		bind					GST-CNP	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_170_4_661_s_65	16103231	(B) Quantitative analysis of tubulin binding to GST-CNP.	bind
12703	1	4112	7	11	NULL	NULL	NULL	tubulin	GP		bind					GST-CNP	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_170_4_661_s_65	16103231	(B) Quantitative analysis of tubulin binding to GST-CNP.	bind
10253	1	4113	5	11	NULL	NULL	NULL	R/M	GP		bind					DNA	NucleicAcid	circular			NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_5_1129_s_104	11741547	(B) R/M bound to the 1.8 kb circular DNA.	bind
12704	1	4113	7	11	NULL	NULL	NULL	R/M	GP		bind					 DNA	NucleicAcid	circular			NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_5_1129_s_104	11741547	(B) R/M bound to the 1.8 kb circular DNA.	bind
10256	1	4114	5	11	NULL	NULL	NULL	Munc18-1 proteins	GP	radiolabelled;;wild-type	bind					GST	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_2_470_s_137	15563604	(B) Radiolabeled Munc18-1  wild-type and mutant proteins were bound to GST, GST-Mint 2, and GST-Mint1 residues  226-314 immobilized on glutathione-Sepharose.	bind
10257	2	4114	5	11	NULL	NULL	NULL	Munc18-1 proteins	GP	radiolabelled;;mutant	bind					GST	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_2_470_s_137	15563604	(B) Radiolabeled Munc18-1  wild-type and mutant proteins were bound to GST, GST-Mint 2, and GST-Mint1 residues  226-314 immobilized on glutathione-Sepharose.	bind
10258	3	4114	5	11	NULL	NULL	NULL	Munc18-1 proteins	GP	radiolabelled;;wild-type	bind					GST-Mint 2	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_2_470_s_137	15563604	(B) Radiolabeled Munc18-1  wild-type and mutant proteins were bound to GST, GST-Mint 2, and GST-Mint1 residues  226-314 immobilized on glutathione-Sepharose.	bind
10259	4	4114	5	11	NULL	NULL	NULL	Munc18-1 proteins	GP	radiolabelled;;mutant	bind					GST-Mint 2	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_2_470_s_137	15563604	(B) Radiolabeled Munc18-1  wild-type and mutant proteins were bound to GST, GST-Mint 2, and GST-Mint1 residues  226-314 immobilized on glutathione-Sepharose.	bind
10260	5	4114	5	11	NULL	NULL	NULL	Munc18-1 proteins	GP	radiolabelled;;wild-type	bind					GST-Mint1	GP	immobilized	226-314		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_2_470_s_137	15563604	(B) Radiolabeled Munc18-1  wild-type and mutant proteins were bound to GST, GST-Mint 2, and GST-Mint1 residues  226-314 immobilized on glutathione-Sepharose.	bind
10261	6	4114	5	11	NULL	NULL	NULL	Munc18-1 proteins	GP	radiolabelled;;mutant	bind					GST-Mint1	GP	immobilized	226-314		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_2_470_s_137	15563604	(B) Radiolabeled Munc18-1  wild-type and mutant proteins were bound to GST, GST-Mint 2, and GST-Mint1 residues  226-314 immobilized on glutathione-Sepharose.	bind
12705	1	4114	7	11	NULL	NULL	NULL	Munc18-1	GP	radiolabeled;;wild-type	bind					GST	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_2_470_s_137	15563604	(B) Radiolabeled Munc18-1  wild-type and mutant proteins were bound to GST, GST-Mint 2, and GST-Mint1 residues  226-314 immobilized on glutathione-Sepharose.	bind
12706	2	4114	7	11	NULL	NULL	NULL	Munc18-1	GP	radiolabeled;;wild-type	bind					GST-Mint 2	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_2_470_s_137	15563604	(B) Radiolabeled Munc18-1  wild-type and mutant proteins were bound to GST, GST-Mint 2, and GST-Mint1 residues  226-314 immobilized on glutathione-Sepharose.	bind
12707	3	4114	7	11	NULL	NULL	NULL	Munc18-1	GP	radiolabeled;;wild-type	bind					GST-Mint1	GP	immobilized	226-314		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_2_470_s_137	15563604	(B) Radiolabeled Munc18-1  wild-type and mutant proteins were bound to GST, GST-Mint 2, and GST-Mint1 residues  226-314 immobilized on glutathione-Sepharose.	bind
12708	4	4114	7	11	NULL	NULL	NULL	Munc18-1	GP	radiolabeled;;mutant	bind					GST	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_2_470_s_137	15563604	(B) Radiolabeled Munc18-1  wild-type and mutant proteins were bound to GST, GST-Mint 2, and GST-Mint1 residues  226-314 immobilized on glutathione-Sepharose.	bind
12709	5	4114	7	11	NULL	NULL	NULL	Munc18-1	GP	radiolabeled;;mutant	bind					GST-Mint 2	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_2_470_s_137	15563604	(B) Radiolabeled Munc18-1  wild-type and mutant proteins were bound to GST, GST-Mint 2, and GST-Mint1 residues  226-314 immobilized on glutathione-Sepharose.	bind
12710	6	4114	7	11	NULL	NULL	NULL	Munc18-1	GP	radiolabeled;;mutant	bind					GST-Mint 1	GP	immobilized	226-314		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_2_470_s_137	15563604	(B) Radiolabeled Munc18-1  wild-type and mutant proteins were bound to GST, GST-Mint 2, and GST-Mint1 residues  226-314 immobilized on glutathione-Sepharose.	bind
10254	1	4115	5	11	NULL	NULL	NULL	CRT	GP		bind								DBD		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6286_s_135	12167720	(B) RanGTP is not a cofactor for CRT binding to the DBD.	bind
10255	2	4115	5	11	NULL	NULL	NULL	RanGTP 	Chemical		is not a cofactor for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6286_s_135	12167720	(B) RanGTP is not a cofactor for CRT binding to the DBD.	bind
12711	1	4115	7	11	NULL	NULL	NULL	CRT	GP		bind					DBD	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6286_s_135	12167720	(B) RanGTP is not a cofactor for CRT binding to the DBD.	bind
12712	2	4115	7	11	NULL	NULL	NULL	RanGTP	Chemical		is not a cofactor for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6286_s_135	12167720	(B) RanGTP is not a cofactor for CRT binding to the DBD.	bind
10262	1	4117	5	11	NULL	NULL	NULL	rec-Pin1	GP		bind					neuronal nuclei	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_expneurol_199_2_328_s_136	16480979	(b) Rec-Pin1 binding: levels of rec-Pin1 binding to neuronal nuclei (Nu;  black bars), cytoplasm (Cyt; grey bars), and lipofuscin granules (Lipo; white bars).	bind
10263	2	4117	5	11	NULL	NULL	NULL	rec-Pin1	GP		bind					neuronal cytoplasm	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_expneurol_199_2_328_s_136	16480979	(b) Rec-Pin1 binding: levels of rec-Pin1 binding to neuronal nuclei (Nu;  black bars), cytoplasm (Cyt; grey bars), and lipofuscin granules (Lipo; white bars).	bind
10264	3	4117	5	11	NULL	NULL	NULL	rec-Pin1	GP		bind					neuronal lipofuscin granules	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_expneurol_199_2_328_s_136	16480979	(b) Rec-Pin1 binding: levels of rec-Pin1 binding to neuronal nuclei (Nu;  black bars), cytoplasm (Cyt; grey bars), and lipofuscin granules (Lipo; white bars).	bind
12713	1	4117	7	11	NULL	NULL	NULL	rec-Pin1 	GP		bind					neuronal nuclei	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_expneurol_199_2_328_s_136	16480979	(b) Rec-Pin1 binding: levels of rec-Pin1 binding to neuronal nuclei (Nu;  black bars), cytoplasm (Cyt; grey bars), and lipofuscin granules (Lipo; white bars).	bind
12714	2	4117	7	11	NULL	NULL	NULL	rec-Pin1 	GP		bind					neuronal cytoplasm	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_expneurol_199_2_328_s_136	16480979	(b) Rec-Pin1 binding: levels of rec-Pin1 binding to neuronal nuclei (Nu;  black bars), cytoplasm (Cyt; grey bars), and lipofuscin granules (Lipo; white bars).	bind
12715	3	4117	7	11	NULL	NULL	NULL	rec-Pin1 	GP		bind					lipofuscin granules	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_expneurol_199_2_328_s_136	16480979	(b) Rec-Pin1 binding: levels of rec-Pin1 binding to neuronal nuclei (Nu;  black bars), cytoplasm (Cyt; grey bars), and lipofuscin granules (Lipo; white bars).	bind
10271	1	4118	5	11	NULL	NULL	NULL	IRP1	GP	recombinant;;Manduca	bind					ferritin	GP	human		IRE transcripts	NULL		NULL	NULL	NULL	NULL	gw60_insectbiochemmolbiol_32_1_85_s_188	11719072	(B) Recombinant  Manduca IRP1 binds human ferritin IRE transcripts.	bind
44477	1	4118	7	11	NULL	NULL	NULL	IRP1	GP	recombinant;;Manduca	bind					ferritin	GP	human		IRE	NULL		NULL	NULL	NULL	NULL	gw60_insectbiochemmolbiol_32_1_85_s_188	11719072	(B) Recombinant  Manduca IRP1 binds human ferritin IRE transcripts.	bind
10279	1	4119	5	11	NULL	NULL	NULL	IRF-3	GP	recombinant	bind			N-terminal		RANTES probe	GP			ISRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_2_959_s_143	9891032	(B) Recombinant N-terminal IRF-3 binds to the RANTES ISRE probe.	bind
12742	1	4119	7	11	NULL	NULL	NULL	IRF-3 	GP	recombinant	binds			N-terminal		RANTES 	GP			ISRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_2_959_s_143	9891032	(B) Recombinant N-terminal IRF-3 binds to the RANTES ISRE probe.	bind
10267	1	4121	5	11	NULL	NULL	NULL	RuBisCo	GP		bind					EL229C-B	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_138	11672529	(B) Refolding of 0.5 muM RuBisCo  bound to EL229C-B with the addition of  either 5 muM SA (.)	bind
10268	2	4121	5	11	NULL	NULL	NULL	SA	Chemical	addition of	refolds					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_138	11672529	(B) Refolding of 0.5 muM RuBisCo  bound to EL229C-B with the addition of  either 5 muM SA (.)	bind
12743	1	4121	7	11	NULL	NULL	NULL	RuBisCo	GP		bind					EL229C-B	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_138	11672529	(B) Refolding of 0.5 muM RuBisCo  bound to EL229C-B with the addition of  either 5 muM SA (.)	bind
12744	2	4121	7	11	NULL	NULL	NULL	statement 1	Process	refolding of 	after addition of					SA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_138	11672529	(B) Refolding of 0.5 muM RuBisCo  bound to EL229C-B with the addition of  either 5 muM SA (.)	bind
10280	1	4122	5	11	NULL	NULL	NULL	RelA	GP		bind					Cyclin T1	GP		cyclin box		NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_2_327_s_102	11545735	(B) RelA binds to the cyclin box of Cyclin T1.	bind
12745	1	4122	7	11	NULL	NULL	NULL	RelA	GP		bind					Cyclin T1	GP		cyclin box		NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_2_327_s_102	11545735	(B) RelA binds to the cyclin box of Cyclin T1.	bind
10281	1	4124	5	11	NULL	NULL	NULL	ResD	GP		does not bind					yclJ	GP	mutations in		promoters putative ResD box	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_19_6477_s_193	15375128	(B) ResD does not bind to  yclJ promoters carrying mutations in the putative ResD box.	bind
12746	1	4124	7	11	NULL	NULL	NULL	ResD	GP		does not bind					 yclJ	GP	mutant		putative ResD box promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_19_6477_s_193	15375128	(B) ResD does not bind to  yclJ promoters carrying mutations in the putative ResD box.	bind
10336	1	4125	5	11	NULL	NULL	NULL	TCR	GP		bind					P6A/HLA-A2	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_13_4_475_s_54	11070166	(B) Residuals for TCR binding to P6A/HLA-A2 assuming no interaction (circles, 3.2  M TCR + 3.3  M P6A/HLA-A2, representing 1.4% complex; triangles, 9.3  M TCR + 9.5  M P6A/HLA-A2, representing 3.6% complex).	bind
12747	1	4125	7	11	NULL	NULL	NULL	TCR	GP		bind					P6A/HLA-A2	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_13_4_475_s_54	11070166	(B) Residuals for TCR binding to P6A/HLA-A2 assuming no interaction (circles, 3.2  M TCR + 3.3  M P6A/HLA-A2, representing 1.4% complex; triangles, 9.3  M TCR + 9.5  M P6A/HLA-A2, representing 3.6% complex).	bind
10343	1	4126	5	11	NULL	NULL	NULL	CodY	GP		bind									fla/chePA promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_10_3118_s_199	12730172	(B) Results of CodY binding to  fla/chePA, the sigmaA-dependent promoter.	bind
13002	2	4126	5	11	NULL	NULL	NULL				is dependent on				fla/chePA	sigmaA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_10_3118_s_199	12730172	(B) Results of CodY binding to  fla/chePA, the sigmaA-dependent promoter.	bind
12748	1	4126	7	11	NULL	NULL	NULL	CodY	GP		bind									fla/chePA promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_10_3118_s_199	12730172	(B) Results of CodY binding to  fla/chePA, the sigmaA-dependent promoter.	bind
12749	2	4126	7	11	NULL	NULL	NULL				is dependent on				fla/chePA	sigmaA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_10_3118_s_199	12730172	(B) Results of CodY binding to  fla/chePA, the sigmaA-dependent promoter.	bind
10385	1	4127	5	11	NULL	NULL	NULL	RFC (p140)	GP		bind					RelA	GP		RHD		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_2_721_s_110	12509469	(B) RFC (p140) binds the RHD of RelA.	bind
12750	1	4127	7	11	NULL	NULL	NULL	RFC (p140)	GP		binds					RelA	GP		RHD		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_2_721_s_110	12509469	(B) RFC (p140) binds the RHD of RelA.	bind
10386	1	4128	5	11	NULL	NULL	NULL	RFXANK	GP		bind					RFXAP	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4455_s_108	10825209	(B) RFXANK binds to RFXAP but not to RFX5 in vitro.	bind
10387	2	4128	5	11	NULL	NULL	NULL	RFXANK	GP		does not bind					RFX5	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4455_s_108	10825209	(B) RFXANK binds to RFXAP but not to RFX5 in vitro.	bind
12752	1	4128	7	11	NULL	NULL	NULL	RFXANK	GP		binds					RFXAP	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4455_s_108	10825209	(B) RFXANK binds to RFXAP but not to RFX5 in vitro.	bind
12753	2	4128	7	11	NULL	NULL	NULL	RFXANK	GP		does not bind					RFX5	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4455_s_108	10825209	(B) RFXANK binds to RFXAP but not to RFX5 in vitro.	bind
10388	1	4129	5	11	NULL	NULL	NULL	GST-Rhotekin	GP		bind		only			Rho-GTP	GP	active			NULL		NULL	NULL	NULL	NULL	gw60_devcell_2_6_733_s_142	12062086	(B) Rho activation assay: after normalization of cell lysates from the conditions shown by anti-Rho Western blot, the lysates were probed with GST-Rhotekin, which only binds active Rho-GTP.	bind
12754	1	4129	7	11	NULL	NULL	NULL	GST-Rhotekin	GP		binds		only			Rho-GTP	GP	active			NULL		NULL	NULL	NULL	NULL	gw60_devcell_2_6_733_s_142	12062086	(B) Rho activation assay: after normalization of cell lysates from the conditions shown by anti-Rho Western blot, the lysates were probed with GST-Rhotekin, which only binds active Rho-GTP.	bind
10389	1	4130	5	11	NULL	NULL	NULL	rIB2	GP		bind					MLK3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4073_s_197	12024021	(B) rIB2 binds to MLK3.	bind
12755	1	4130	7	11	NULL	NULL	NULL	 rIB2	GP		binds to					MLK3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4073_s_197	12024021	(B) rIB2 binds to MLK3.	bind
10390	1	4131	5	11	NULL	NULL	NULL	CksHs1	GP		bind					CDK2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_84_6_863_s_36	8601310	(B) Ribbon diagram  of CksHs1 (yellow) bound to CDK2, with the N-lobe in purple and the C-lobe  in blue and green.	bind
12756	1	4131	7	11	NULL	NULL	NULL	CksHs1	GP		bind					CDK2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_84_6_863_s_36	8601310	(B) Ribbon diagram  of CksHs1 (yellow) bound to CDK2, with the N-lobe in purple and the C-lobe  in blue and green.	bind
10391	1	4132	5	11	NULL	NULL	NULL	HSA	Chemical		is saturated with					palmitic acid	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1688_2_102_s_126	14990340	(B) Rifampin binding to HSA saturated  with palmitic acid.	bind
10392	2	4132	5	11	NULL	NULL	NULL	Rifampin	Chemical		bind					statement 1	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1688_2_102_s_126	14990340	(B) Rifampin binding to HSA saturated  with palmitic acid.	bind
12758	1	4132	7	11	NULL	NULL	NULL	HSA	Chemical		is saturated with					palmitic acid	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1688_2_102_s_126	14990340	(B) Rifampin binding to HSA saturated  with palmitic acid.	bind
12759	2	4132	7	11	NULL	NULL	NULL	Rifampin	Chemical		bind					statement 1	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1688_2_102_s_126	14990340	(B) Rifampin binding to HSA saturated  with palmitic acid.	bind
10393	1	4133	5	11	NULL	NULL	NULL	chromaffin cell cytoplasmic protein	GP		bind					TH mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_120_2_91_s_151	14741398	(B) RNA-EMSA of chromaffin cell cytoplasmic protein binding to TH mRNA.  32P-labeled RNA probes THC, TH1, TH2 and TH3 were incubated alone (lanes 1,3,5 and 7)  or with 40  g S100 cytoplasmic extracts (lanes 2, 4, 6 and 8) and separated on non-denaturing  gels.	bind
12777	1	4133	7	11	NULL	NULL	NULL	chromaffin cell cytoplasmic protein	GP		bind					TH mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_120_2_91_s_151	14741398	(B) RNA-EMSA of chromaffin cell cytoplasmic protein binding to TH mRNA.  32P-labeled RNA probes THC, TH1, TH2 and TH3 were incubated alone (lanes 1,3,5 and 7)  or with 40  g S100 cytoplasmic extracts (lanes 2, 4, 6 and 8) and separated on non-denaturing  gels.	bind
10400	1	4134	5	11	NULL	NULL	NULL	cyclin T protein	GP	GST-cleaved	bind					TAR-2 RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_188	9491887	(B) RNase footprint analysis of the binding  of GST-cleaved cyclin T and GST-Tat-2 (aa 1 - 99) proteins to TAR-2 RNA.	bind
10401	2	4134	5	11	NULL	NULL	NULL	GST-Tat-2 protein	GP		bind			aa 1 - 99		TAR-2 RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_188	9491887	(B) RNase footprint analysis of the binding  of GST-cleaved cyclin T and GST-Tat-2 (aa 1 - 99) proteins to TAR-2 RNA.	bind
12760	1	4134	7	11	NULL	NULL	NULL	 cyclin T	GP	GST-cleaved	bind					TAR-2 RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_188	9491887	(B) RNase footprint analysis of the binding  of GST-cleaved cyclin T and GST-Tat-2 (aa 1 - 99) proteins to TAR-2 RNA.	bind
12761	2	4134	7	11	NULL	NULL	NULL	GST-Tat-2	GP		bind			1 - 99		TAR-2 RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_92_4_451_s_188	9491887	(B) RNase footprint analysis of the binding  of GST-cleaved cyclin T and GST-Tat-2 (aa 1 - 99) proteins to TAR-2 RNA.	bind
10403	1	4135	5	11	NULL	NULL	NULL	Robo1	GP		bind		specifically			srGAPs	GP		SH3 domains		NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_209_s_98	11672528	(B) Robo1 specifically binds to SH3 domains  in srGAPs but not to SH3 motif  in Src or Graf.	bind
10404	2	4135	5	11	NULL	NULL	NULL	Robo1	GP		does not bind					Src	GP		SH3 motif		NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_209_s_98	11672528	(B) Robo1 specifically binds to SH3 domains  in srGAPs but not to SH3 motif  in Src or Graf.	bind
10406	3	4135	5	11	NULL	NULL	NULL	Robo1	GP		does not bind					Graf	GP		SH3 motif		NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_209_s_98	11672528	(B) Robo1 specifically binds to SH3 domains  in srGAPs but not to SH3 motif  in Src or Graf.	bind
10407	4	4135	5	11	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_209_s_98	11672528	(B) Robo1 specifically binds to SH3 domains  in srGAPs but not to SH3 motif  in Src or Graf.	bind
12762	1	4135	7	11	NULL	NULL	NULL	Robo1	GP		binds		specifically			srGAPs	GP		SH3		NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_209_s_98	11672528	(B) Robo1 specifically binds to SH3 domains  in srGAPs but not to SH3 motif  in Src or Graf.	bind
12763	2	4135	7	11	NULL	NULL	NULL	Robo1	GP		does not bind					Src	GP		SH3 moif		NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_209_s_98	11672528	(B) Robo1 specifically binds to SH3 domains  in srGAPs but not to SH3 motif  in Src or Graf.	bind
12764	3	4135	7	11	NULL	NULL	NULL	Robo1	GP		does not bind					Graf	GP		SH3 moif		NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_209_s_98	11672528	(B) Robo1 specifically binds to SH3 domains  in srGAPs but not to SH3 motif  in Src or Graf.	bind
10409	1	4136	5	11	NULL	NULL	NULL	CBP	GP		enhance					GCMa	GP	transcriptional activity of	C-terminal TAD		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8401_s_336	16166624	(B) Roles of lysine367, lysine406, and lysine409 in the CBP-enhanced transcriptional activity of GCMa C-terminal TAD. CV1 cells were  transfected with different combinations of 0.5 mug of pGal4-GCMa-Flag(300-436), pGal4-GCMa-Flag(300-436)K2R,  pGal4-GCMa-Flag(300-436)K3R, and pCBP-HA.	bind
12765	1	4136	7	11	NULL	NULL	NULL	CBP	GP		enhance					GCMa	GP	transcriptional activity of	C-terminal TAD		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8401_s_336	16166624	(B) Roles of lysine367, lysine406, and lysine409 in the CBP-enhanced transcriptional activity of GCMa C-terminal TAD. CV1 cells were  transfected with different combinations of 0.5 mug of pGal4-GCMa-Flag(300-436), pGal4-GCMa-Flag(300-436)K2R,  pGal4-GCMa-Flag(300-436)K3R, and pCBP-HA.	bind
10411	1	4137	5	11	NULL	NULL	NULL	PABPC1	GP		bind					Gl pre-mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_8_3085_s_179	16581783	(B) RT-PCR of Gl pre-mRNA  from intron 1 into intron 2 (introns 1 and 2) and MUP mRNA to determine the extent  of PABPC1 binding to Gl pre-mRNA that occurs after cell lysis.	bind
10412	2	4137	5	11	NULL	NULL	NULL	statement 1	Process		occurs after					cell lysis	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_8_3085_s_179	16581783	(B) RT-PCR of Gl pre-mRNA  from intron 1 into intron 2 (introns 1 and 2) and MUP mRNA to determine the extent  of PABPC1 binding to Gl pre-mRNA that occurs after cell lysis.	bind
12766	1	4137	7	11	NULL	NULL	NULL	PABPC1	GP		bind					Gl pre-mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_8_3085_s_179	16581783	(B) RT-PCR of Gl pre-mRNA  from intron 1 into intron 2 (introns 1 and 2) and MUP mRNA to determine the extent  of PABPC1 binding to Gl pre-mRNA that occurs after cell lysis.	bind
12767	2	4137	7	11	NULL	NULL	NULL	statement 1	Process		occurs after					cell lysis	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_8_3085_s_179	16581783	(B) RT-PCR of Gl pre-mRNA  from intron 1 into intron 2 (introns 1 and 2) and MUP mRNA to determine the extent  of PABPC1 binding to Gl pre-mRNA that occurs after cell lysis.	bind
10414	1	4139	5	11	NULL	NULL	NULL	sAPP695T	GP		bind					HK cleavage products	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1571_3_225_s_276	12090937	(B) sAPP695T binding to the HK cleavage products.	bind
12768	1	4139	7	11	NULL	NULL	NULL	sAPP695T 	GP		bind					HK cleavage products	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1571_3_225_s_276	12090937	(B) sAPP695T binding to the HK cleavage products.	bind
10415	1	4140	5	11	NULL	NULL	NULL	SATB1	GP		bind					IL-2 	GP			promoter	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1620_s_178	15713622	(B) SATB1 binds to the IL-2 promoter in vitro.	bind
12769	1	4140	7	11	NULL	NULL	NULL	 SATB1	GP		binds					 IL-2	GP			promoter	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1620_s_178	15713622	(B) SATB1 binds to the IL-2 promoter in vitro.	bind
10416	1	4142	5	11	NULL	NULL	NULL	[3]R-PIA	GP		bind		specifically			A1Rs	GP	purified			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_14_5164_s_242	10866672	(B) Saturation isotherm of [3]R-PIA specific binding to purified A1Rs in the absence or presence of 30 nM hsc73.	bind
12770	1	4142	7	11	NULL	NULL	NULL	[3]R-PIA	GP		bind		specifically			A1Rs	GP	purified			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_14_5164_s_242	10866672	(B) Saturation isotherm of [3]R-PIA specific binding to purified A1Rs in the absence or presence of 30 nM hsc73.	bind
10417	1	4143	5	11	NULL	NULL	NULL	sbp1p	GP		bind					spi1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_genetics_148_2_645_s_186	9504913	(B) sbp1p binds to spi1p.	bind
12771	1	4143	7	11	NULL	NULL	NULL	sbp1p	GP		binds to					spi1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_genetics_148_2_645_s_186	9504913	(B) sbp1p binds to spi1p.	bind
10418	1	4144	5	11	NULL	NULL	NULL	sc1	GP		bind					FMRP proteins	GP		N terminus		NULL		NULL	NULL	NULL	NULL	gw60_cell_107_4_489_s_141	11719189	(B) sc1 binding to FMRP  N and C termini fusion proteins (see  Experimental Procedures).	bind
10419	2	4144	5	11	NULL	NULL	NULL	sc1	GP		bind					FMRP proteins	GP		C terminus		NULL		NULL	NULL	NULL	NULL	gw60_cell_107_4_489_s_141	11719189	(B) sc1 binding to FMRP  N and C termini fusion proteins (see  Experimental Procedures).	bind
44428	3	4144	5	11	NULL	NULL	NULL	FMRP	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_4_489_s_141	11719189	(B) sc1 binding to FMRP  N and C termini fusion proteins (see  Experimental Procedures).	bind
12772	1	4144	7	11	NULL	NULL	NULL	sc1 	GP		bind					FMRP  protein	GP		N terminus		NULL		NULL	NULL	NULL	NULL	gw60_cell_107_4_489_s_141	11719189	(B) sc1 binding to FMRP  N and C termini fusion proteins (see  Experimental Procedures).	bind
12773	2	4144	7	11	NULL	NULL	NULL	sc1 	GP		bind					FMRP  protein	GP		C terminus		NULL		NULL	NULL	NULL	NULL	gw60_cell_107_4_489_s_141	11719189	(B) sc1 binding to FMRP  N and C termini fusion proteins (see  Experimental Procedures).	bind
10452	1	4145	5	11	NULL	NULL	NULL	YFP- lac rep-SRC570-780 protein	GP		bind									lac operator sequences	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_10_3437_s_84	11971975	(B) Schematic of the YFP- lac rep-SRC570-780 fusion protein, which binds to  lac operator sequences and can recruit wild-type ER or CFP-ER.	bind
10453	2	4145	5	11	NULL	NULL	NULL	statement 1	Process		recruit					ER	GP	wild-type			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_10_3437_s_84	11971975	(B) Schematic of the YFP- lac rep-SRC570-780 fusion protein, which binds to  lac operator sequences and can recruit wild-type ER or CFP-ER.	bind
10454	3	4145	5	11	NULL	NULL	NULL	statement 1	Process		recruit					CFP-ER	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_10_3437_s_84	11971975	(B) Schematic of the YFP- lac rep-SRC570-780 fusion protein, which binds to  lac operator sequences and can recruit wild-type ER or CFP-ER.	bind
44429	4	4145	5	11	NULL	NULL	NULL	YFP- lac rep-SRC570-780	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_10_3437_s_84	11971975	(B) Schematic of the YFP- lac rep-SRC570-780 fusion protein, which binds to  lac operator sequences and can recruit wild-type ER or CFP-ER.	bind
12774	1	4145	7	11	NULL	NULL	NULL	YFP- lac rep-SRC570-780	GP		binds									lac operator sequences	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_10_3437_s_84	11971975	(B) Schematic of the YFP- lac rep-SRC570-780 fusion protein, which binds to  lac operator sequences and can recruit wild-type ER or CFP-ER.	bind
12775	2	4145	7	11	NULL	NULL	NULL	statement 1	Process		recruits					ER	GP	wild-type			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_10_3437_s_84	11971975	(B) Schematic of the YFP- lac rep-SRC570-780 fusion protein, which binds to  lac operator sequences and can recruit wild-type ER or CFP-ER.	bind
12776	3	4145	7	11	NULL	NULL	NULL	statement 1	Process		recruits					CFP-ER	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_10_3437_s_84	11971975	(B) Schematic of the YFP- lac rep-SRC570-780 fusion protein, which binds to  lac operator sequences and can recruit wild-type ER or CFP-ER.	bind
44407	4	4145	7	11	NULL	NULL	NULL	YFP- lac rep-SRC570-780	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_10_3437_s_84	11971975	(B) Schematic of the YFP- lac rep-SRC570-780 fusion protein, which binds to  lac operator sequences and can recruit wild-type ER or CFP-ER.	bind
11438	1	4151	5	11	NULL	NULL	NULL	endo-oxabicyclic inhibitor	Chemical		bind					CM	CellComponent	E. coli			NULL		NULL	NULL	NULL	NULL	gw60_structure_5_11_1437_s_96	9384560	(b) Scheme of interactions between the inhibitor and active site residues of YCM.  (c) Stereo view of the binding mode of the inhibitor to the active site in ITRP.  (d,e) Binding of the  endo-oxabicyclic inhibitor to  E. coli CM (d) and to  B. subtilis CM (e).	bind
11439	2	4151	5	11	NULL	NULL	NULL	endo-oxabicyclic inhibitor	Chemical		bind					CM	CellComponent	B. subtilis			NULL		NULL	NULL	NULL	NULL	gw60_structure_5_11_1437_s_96	9384560	(b) Scheme of interactions between the inhibitor and active site residues of YCM.  (c) Stereo view of the binding mode of the inhibitor to the active site in ITRP.  (d,e) Binding of the  endo-oxabicyclic inhibitor to  E. coli CM (d) and to  B. subtilis CM (e).	bind
12880	1	4151	7	11	NULL	NULL	NULL	endo-oxabicyclic inhibitor	Chemical		bind					CM	CellComponent	E.coli			NULL		NULL	NULL	NULL	NULL	gw60_structure_5_11_1437_s_96	9384560	(b) Scheme of interactions between the inhibitor and active site residues of YCM.  (c) Stereo view of the binding mode of the inhibitor to the active site in ITRP.  (d,e) Binding of the  endo-oxabicyclic inhibitor to  E. coli CM (d) and to  B. subtilis CM (e).	bind
12881	2	4151	7	11	NULL	NULL	NULL	endo-oxabicyclic inhibitor	Chemical		bind					CM	CellComponent	B. subtilis			NULL		NULL	NULL	NULL	NULL	gw60_structure_5_11_1437_s_96	9384560	(b) Scheme of interactions between the inhibitor and active site residues of YCM.  (c) Stereo view of the binding mode of the inhibitor to the active site in ITRP.  (d,e) Binding of the  endo-oxabicyclic inhibitor to  E. coli CM (d) and to  B. subtilis CM (e).	bind
10455	1	4153	5	11	NULL	NULL	NULL	EphA3-AP	GP		bind					ephrins-A	GP				NULL	muscle	NULL	NULL	NULL	NULL	gw60_neuron_25_2_295_s_52	10719886	(B) Sections of muscle stained with EphA3-AP or EphA5-Fc fusion proteins, which bind to ephrins-A but not to ephrins-B.	bind
10456	2	4153	5	11	NULL	NULL	NULL	EphA3-AP	GP		does not bind					ephrins-B	GP				NULL	muscle	NULL	NULL	NULL	NULL	gw60_neuron_25_2_295_s_52	10719886	(B) Sections of muscle stained with EphA3-AP or EphA5-Fc fusion proteins, which bind to ephrins-A but not to ephrins-B.	bind
10457	3	4153	5	11	NULL	NULL	NULL	EphA5-Fc	GP		bind					ephrins-A	GP				NULL	muscle	NULL	NULL	NULL	NULL	gw60_neuron_25_2_295_s_52	10719886	(B) Sections of muscle stained with EphA3-AP or EphA5-Fc fusion proteins, which bind to ephrins-A but not to ephrins-B.	bind
10458	4	4153	5	11	NULL	NULL	NULL	EphA5-Fc	GP		does not bind					ephrins-B	GP				NULL	muscle	NULL	NULL	NULL	NULL	gw60_neuron_25_2_295_s_52	10719886	(B) Sections of muscle stained with EphA3-AP or EphA5-Fc fusion proteins, which bind to ephrins-A but not to ephrins-B.	bind
10459	5	4153	5	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_25_2_295_s_52	10719886	(B) Sections of muscle stained with EphA3-AP or EphA5-Fc fusion proteins, which bind to ephrins-A but not to ephrins-B.	bind
10460	6	4153	5	11	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_25_2_295_s_52	10719886	(B) Sections of muscle stained with EphA3-AP or EphA5-Fc fusion proteins, which bind to ephrins-A but not to ephrins-B.	bind
44430	7	4153	5	11	NULL	NULL	NULL	EphA3-AP	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_25_2_295_s_52	10719886	(B) Sections of muscle stained with EphA3-AP or EphA5-Fc fusion proteins, which bind to ephrins-A but not to ephrins-B.	bind
44431	8	4153	5	11	NULL	NULL	NULL	EphA5-Fc	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_25_2_295_s_52	10719886	(B) Sections of muscle stained with EphA3-AP or EphA5-Fc fusion proteins, which bind to ephrins-A but not to ephrins-B.	bind
12883	1	4153	7	11	NULL	NULL	NULL	EphA3-AP	GP		bind					ephrins-A 	GP				NULL	muscle	NULL	NULL	NULL	NULL	gw60_neuron_25_2_295_s_52	10719886	(B) Sections of muscle stained with EphA3-AP or EphA5-Fc fusion proteins, which bind to ephrins-A but not to ephrins-B.	bind
12884	2	4153	7	11	NULL	NULL	NULL	EphA5-Fc	GP		bind					ephrins-A 	GP				NULL	muscle	NULL	NULL	NULL	NULL	gw60_neuron_25_2_295_s_52	10719886	(B) Sections of muscle stained with EphA3-AP or EphA5-Fc fusion proteins, which bind to ephrins-A but not to ephrins-B.	bind
12885	3	4153	7	11	NULL	NULL	NULL	EphA3-AP	GP		does not bind					ephrins-B	GP				NULL	muscle	NULL	NULL	NULL	NULL	gw60_neuron_25_2_295_s_52	10719886	(B) Sections of muscle stained with EphA3-AP or EphA5-Fc fusion proteins, which bind to ephrins-A but not to ephrins-B.	bind
12886	4	4153	7	11	NULL	NULL	NULL	EphA5-Fc	GP		does not bind					ephrins-B	GP				NULL	muscle	NULL	NULL	NULL	NULL	gw60_neuron_25_2_295_s_52	10719886	(B) Sections of muscle stained with EphA3-AP or EphA5-Fc fusion proteins, which bind to ephrins-A but not to ephrins-B.	bind
44408	5	4153	7	11	NULL	NULL	NULL	EphA3-AP	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_25_2_295_s_52	10719886	(B) Sections of muscle stained with EphA3-AP or EphA5-Fc fusion proteins, which bind to ephrins-A but not to ephrins-B.	bind
44479	6	4153	7	11	NULL	NULL	NULL	EphA5-Fc	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_25_2_295_s_52	10719886	(B) Sections of muscle stained with EphA3-AP or EphA5-Fc fusion proteins, which bind to ephrins-A but not to ephrins-B.	bind
54280	7	4153	7	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_25_2_295_s_52	10719886	(B) Sections of muscle stained with EphA3-AP or EphA5-Fc fusion proteins, which bind to ephrins-A but not to ephrins-B.	bind
54281	8	4153	7	11	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_25_2_295_s_52	10719886	(B) Sections of muscle stained with EphA3-AP or EphA5-Fc fusion proteins, which bind to ephrins-A but not to ephrins-B.	bind
10461	1	4154	5	11	NULL	NULL	NULL	VASP	GP	eukaryotic;;recombinant	bind					F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_144_6_1245_s_325	10087267	(b) Sedimentation assay for the  binding of eukaryotic recombinant VASP to F-actin.	bind
44478	1	4154	7	11	NULL	NULL	NULL	VASP	GP	eukaryotic;;recombinant	bind					F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_144_6_1245_s_325	10087267	(b) Sedimentation assay for the  binding of eukaryotic recombinant VASP to F-actin.	bind
10462	1	4155	5	11	NULL	NULL	NULL	CSL	GP		bind					Caco-2 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_10_5282_s_235	10496907	(B) Self-displaceable binding of CSL to Caco-2 cells.	bind
12888	1	4155	7	11	NULL	NULL	NULL	CSL	GP		bind					Caco-2 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_10_5282_s_235	10496907	(B) Self-displaceable binding of CSL to Caco-2 cells.	bind
10463	1	4158	5	11	NULL	NULL	NULL	p53	GP		bind		sequence specific			DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_267	14612423	(B) Sequence-specific DNA binding changes the conformation of p53 ( ), thus permitting acetylation to occur in a PXXP-dependent manner.	bind
10464	2	4158	5	11	NULL	NULL	NULL	statement 1	Process		change					p53	GP	conformation of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_267	14612423	(B) Sequence-specific DNA binding changes the conformation of p53 ( ), thus permitting acetylation to occur in a PXXP-dependent manner.	bind
10465	3	4158	5	11	NULL	NULL	NULL	statement 2	Process		permit					p53	GP	acetylation of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_267	14612423	(B) Sequence-specific DNA binding changes the conformation of p53 ( ), thus permitting acetylation to occur in a PXXP-dependent manner.	bind
10466	4	4158	5	11	NULL	NULL	NULL	statement 3	Process		is dependent on								PXXP		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_267	14612423	(B) Sequence-specific DNA binding changes the conformation of p53 ( ), thus permitting acetylation to occur in a PXXP-dependent manner.	bind
12890	1	4158	7	11	NULL	NULL	NULL	p53	GP		bind		sequence-specific			DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_267	14612423	(B) Sequence-specific DNA binding changes the conformation of p53 ( ), thus permitting acetylation to occur in a PXXP-dependent manner.	bind
12891	2	4158	7	11	NULL	NULL	NULL	statement 1	Process		changes					p53	GP	conformation of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_267	14612423	(B) Sequence-specific DNA binding changes the conformation of p53 ( ), thus permitting acetylation to occur in a PXXP-dependent manner.	bind
12892	3	4158	7	11	NULL	NULL	NULL	statement 2	Process		permits					p53	GP	acetylation of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_267	14612423	(B) Sequence-specific DNA binding changes the conformation of p53 ( ), thus permitting acetylation to occur in a PXXP-dependent manner.	bind
16307	4	4158	7	11	NULL	NULL	NULL	statement 3	Process		is dependent on								PXXP		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_267	14612423	(B) Sequence-specific DNA binding changes the conformation of p53 ( ), thus permitting acetylation to occur in a PXXP-dependent manner.	bind
11440	1	4161	5	11	NULL	NULL	NULL	diazepam	Chemical		bind					HSA	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1750_1_93_s_169	15890566	(B) shows the binding isotherm of diazepam to  HSA as a function of GnHCl concentration at a fixed diazepam/albumin molar ratio  of 2:1.	bind
12893	1	4161	7	NULL	NULL	0	NULL	diazepam	NULL		bind	NULL				HSA	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1750_1_93_s_169	15890566	(B) shows the binding isotherm of diazepam to  HSA as a function of GnHCl concentration at a fixed diazepam/albumin molar ratio  of 2:1.	bind
10467	1	4162	5	11	NULL	NULL	NULL	HoxB1 peptide	GP		bind					Pbx1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_96_4_587_s_116	10052460	(B) Side  view of the HoxB1 peptide bound to Pbx1.	bind
12894	1	4162	7	11	NULL	NULL	NULL	HoxB1 peptide	GP		bind					Pbx1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_96_4_587_s_116	10052460	(B) Side  view of the HoxB1 peptide bound to Pbx1.	bind
10468	1	4163	5	11	NULL	NULL	NULL	Ni2+	Chemical		bind					HypA	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_3_726_s_145	12533448	(B) Sigmoidal curve for Ni2+ binding by HypA (wild type).	bind
12895	1	4163	7	11	NULL	NULL	NULL	Ni2+	Chemical		bind					HypA	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_3_726_s_145	12533448	(B) Sigmoidal curve for Ni2+ binding by HypA (wild type).	bind
10469	1	4165	5	11	NULL	NULL	NULL	O2	Chemical		bind					heme a3	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1503_3_261_s_93	11115638	(B) Simulated curves for O2 binding to heme  a3 with a second-order rate constant of 108 M-1s-1, limited by the CO-off rate from CuB (different values of  koff c.f.  kmax in  Eq. 1).	bind
12896	1	4165	7	11	NULL	NULL	NULL	O2	Chemical		bind					heme a3	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1503_3_261_s_93	11115638	(B) Simulated curves for O2 binding to heme  a3 with a second-order rate constant of 108 M-1s-1, limited by the CO-off rate from CuB (different values of  koff c.f.  kmax in  Eq. 1).	bind
10471	1	4166	5	11	NULL	NULL	NULL	BR-II	GP	singly expressed 	bind		weakly			BMP-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_3_1023_s_208	10712517	(B) Singly expressed BR-II binds the BMP-2 only weakly.	bind
12897	1	4166	7	11	NULL	NULL	NULL	BR-II	GP	Singly expressed	binds		weakly			 BMP-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_3_1023_s_208	10712517	(B) Singly expressed BR-II binds the BMP-2 only weakly.	bind
10472	1	4167	5	11	NULL	NULL	NULL	Skp2	GP		bind		specifically			p27CP	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_12_661_s_72	10375532	(b) Skp2 specifically binds to p27CP.	bind
12898	1	4167	7	11	NULL	NULL	NULL	Skp2	GP		binds		specifically			p27CP	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_12_661_s_72	10375532	(b) Skp2 specifically binds to p27CP.	bind
10473	1	4168	5	11	NULL	NULL	NULL	Snf1	GP		bind					GST-Gln3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_4_1246_s_181	11809814	(B) Snf1 binds to GST-Gln3.	bind
12899	1	4168	7	11	NULL	NULL	NULL	Snf1	GP		bind					GST-Gln3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_4_1246_s_181	11809814	(B) Snf1 binds to GST-Gln3.	bind
10474	1	4169	5	11	NULL	NULL	NULL	PKC	GP	activity of	regulate					SOCE	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_7_1033_s_192	15051735	(B) SOCE is regulated  by PKC activity.	bind
12900	1	4169	7	11	NULL	NULL	NULL	PKC	GP	activity of	regulates					SOCE	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_7_1033_s_192	15051735	(B) SOCE is regulated  by PKC activity.	bind
10475	1	4172	5	11	NULL	NULL	NULL	L1Fc	GP		is					L1	GP	Soluble			NULL		NULL	NULL	NULL	NULL	gw60_embo_21_23_6348_s_127	12456642	(b) Soluble L1 (L1Fc) binds both L1 and NP-1 on the growth cone and switches Sema3A repulsion to attraction.	bind
10476	2	4172	5	11	NULL	NULL	NULL	L1Fc	GP		bind					L1	GP	soluble			NULL	on the growth cone	NULL	NULL	NULL	NULL	gw60_embo_21_23_6348_s_127	12456642	(b) Soluble L1 (L1Fc) binds both L1 and NP-1 on the growth cone and switches Sema3A repulsion to attraction.	bind
10477	3	4172	5	11	NULL	NULL	NULL	L1Fc	GP		bind					NP-1	GP				NULL	on the growth cone	NULL	NULL	NULL	NULL	gw60_embo_21_23_6348_s_127	12456642	(b) Soluble L1 (L1Fc) binds both L1 and NP-1 on the growth cone and switches Sema3A repulsion to attraction.	bind
10478	4	4172	5	11	NULL	NULL	NULL	Sema3A	GP	repulsion of	switches to					Sema3A	GP	attraction of			NULL		NULL	NULL	NULL	NULL	gw60_embo_21_23_6348_s_127	12456642	(b) Soluble L1 (L1Fc) binds both L1 and NP-1 on the growth cone and switches Sema3A repulsion to attraction.	bind
13003	5	4172	5	11	NULL	NULL	NULL	L1	GP	soluble	causes					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_23_6348_s_127	12456642	(b) Soluble L1 (L1Fc) binds both L1 and NP-1 on the growth cone and switches Sema3A repulsion to attraction.	bind
12903	3	4172	7	11	NULL	NULL	NULL	Sema3A	GP	repulsion of	switches to					Sema3A	GP	attraction of			NULL		NULL	NULL	NULL	NULL	gw60_embo_21_23_6348_s_127	12456642	(b) Soluble L1 (L1Fc) binds both L1 and NP-1 on the growth cone and switches Sema3A repulsion to attraction.	bind
12905	5	4172	7	11	NULL	NULL	NULL	L1	GP	soluble	is					L1Fc	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_23_6348_s_127	12456642	(b) Soluble L1 (L1Fc) binds both L1 and NP-1 on the growth cone and switches Sema3A repulsion to attraction.	bind
44480	1	4172	7	11	NULL	NULL	NULL	L1	GP	soluble	bind					L1	GP				NULL	on the growth cone	NULL	NULL	NULL	NULL	gw60_embo_21_23_6348_s_127	12456642	(b) Soluble L1 (L1Fc) binds both L1 and NP-1 on the growth cone and switches Sema3A repulsion to attraction.	bind
44481	2	4172	7	11	NULL	NULL	NULL	L1	GP	soluble	bind					NP-1	GP				NULL	on the growth cone	NULL	NULL	NULL	NULL	gw60_embo_21_23_6348_s_127	12456642	(b) Soluble L1 (L1Fc) binds both L1 and NP-1 on the growth cone and switches Sema3A repulsion to attraction.	bind
44482	4	4172	7	11	NULL	NULL	NULL	L1	GP	soluble	causes					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_23_6348_s_127	12456642	(b) Soluble L1 (L1Fc) binds both L1 and NP-1 on the growth cone and switches Sema3A repulsion to attraction.	bind
10479	1	4174	5	11	NULL	NULL	NULL	Sp proteins	GP		is expressed in		transiently			SL2 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_41_4_583_s_120	10744779	(B) Sp proteins transiently expressed in SL2 cells bind to the  Ctpct probe containing multiple binding elements.	bind
10480	2	4174	5	11	NULL	NULL	NULL	statement 1	GP		bind					Ctpct probe	GP		multiple binding elements		NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_41_4_583_s_120	10744779	(B) Sp proteins transiently expressed in SL2 cells bind to the  Ctpct probe containing multiple binding elements.	bind
12906	1	4174	7	11	NULL	NULL	NULL	SL2 cells	cell		bind					 Ctpct probe	GP		multiple binding elements		NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_41_4_583_s_120	10744779	(B) Sp proteins transiently expressed in SL2 cells bind to the  Ctpct probe containing multiple binding elements.	bind
12907	2	4174	7	11	NULL	NULL	NULL	Sp proteins	GP		 expressed in		transiently			SL2 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_41_4_583_s_120	10744779	(B) Sp proteins transiently expressed in SL2 cells bind to the  Ctpct probe containing multiple binding elements.	bind
10481	1	4176	5	11	NULL	NULL	NULL	Oct-1	GP		bind		specifically							Oct-1 site	NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_1_55_s_123	15527761	(B) Specific binding of Oct-1  to the Oct-1 site.	bind
12908	1	4176	7	11	NULL	NULL	NULL	Oct-1	GP		bind		specifically							Oct-1 site	NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_1_55_s_123	15527761	(B) Specific binding of Oct-1  to the Oct-1 site.	bind
10482	1	4177	5	11	NULL	NULL	NULL	PPARgamma2/RXRalpha	GP		bind		specifically							PPRE	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_3_1313_s_238	14729975	(B) Specific binding of PPARgamma2/RXRalpha to the PPRE. PPARgamma2 and RXRalpha were synthesized in a rabbit reticulocyte lysate system.	bind
12909	1	4177	7	11	NULL	NULL	NULL	PPARgamma2/RXRalpha	GP		bind		specifically							PPRE	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_3_1313_s_238	14729975	(B) Specific binding of PPARgamma2/RXRalpha to the PPRE. PPARgamma2 and RXRalpha were synthesized in a rabbit reticulocyte lysate system.	bind
10483	1	4179	5	11	NULL	NULL	NULL	psi RNA	NucleicAcid		bind					NC protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_4_1181_s_88	15249214	(B) Specific inhibition by aptamer  N70-13 of psi RNA binding to NC protein.	bind
10484	2	4179	5	11	NULL	NULL	NULL	aptamer N70-13	NucleicAcid		inhibit		specifically			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_4_1181_s_88	15249214	(B) Specific inhibition by aptamer  N70-13 of psi RNA binding to NC protein.	bind
12910	1	4179	7	11	NULL	NULL	NULL	psi RNA	NucleicAcid		binds					NC protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_4_1181_s_88	15249214	(B) Specific inhibition by aptamer  N70-13 of psi RNA binding to NC protein.	bind
12911	2	4179	7	11	NULL	NULL	NULL	aptamer N70-13	NucleicAcid		inhibits		specifically			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_4_1181_s_88	15249214	(B) Specific inhibition by aptamer  N70-13 of psi RNA binding to NC protein.	bind
10485	1	4180	5	11	NULL	NULL	NULL	transferrin	GP	specific	bind					L4-L5 fusion	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_2_732_s_218	11796606	(B) Specific transferrin binding to L4-L5 fusion	bind
12912	1	4180	7	11	NULL	NULL	NULL	transferrin	GP	specific	bind					L4-L5 fusion	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_2_732_s_218	11796606	(B) Specific transferrin binding to L4-L5 fusion	bind
10486	1	4181	5	11	NULL	NULL	NULL	SPN	GP		bind					Xpo1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4660_s_90	16030253	(B) SPN binding  to Xpo1 is extremely sensitive to mutation.	bind
10487	2	4181	5	11	NULL	NULL	NULL	statement 1	Process		is sensitive to		extremely			mutation	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4660_s_90	16030253	(B) SPN binding  to Xpo1 is extremely sensitive to mutation.	bind
12913	1	4181	7	11	NULL	NULL	NULL	SPN	GP		bind					Xpo1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4660_s_90	16030253	(B) SPN binding  to Xpo1 is extremely sensitive to mutation.	bind
12914	2	4181	7	11	NULL	NULL	NULL	statement 1	Process		is sensitive to		extremely			mutation	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4660_s_90	16030253	(B) SPN binding  to Xpo1 is extremely sensitive to mutation.	bind
10488	1	4182	5	11	NULL	NULL	NULL	Spt10p	GP		bind		specifically			HTA1-HTB1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_20_9127_s_271	16199888	(B) Spt10p binds specifically  to the  HTA1-HTB1 promoter.	bind
12915	1	4182	7	11	NULL	NULL	NULL	Spt10p	GP		binds		specifically			HTA1-HTB1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_20_9127_s_271	16199888	(B) Spt10p binds specifically  to the  HTA1-HTB1 promoter.	bind
10492	1	4184	5	11	NULL	NULL	NULL	Src	GP		bind					mDia2	GP		proline-rich FH1 domain		NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_1_13_s_57	10678165	(B) Src binds the proline-rich FH1 domain of mDia2.	bind
12919	1	4184	7	11	NULL	NULL	NULL	 Src	GP		bind					mDia2	GP		proline-rich FH1 domain		NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_1_13_s_57	10678165	(B) Src binds the proline-rich FH1 domain of mDia2.	bind
10493	1	4185	5	11	NULL	NULL	NULL	SREBP-1a	GP		bind					CBP/p300	GP	full-length	KIX domain		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_10_3392_s_114	12724399	(B) SREBP-1a binding to the KIX domain of full-length CBP/p300 prevents binding of the coactivators to the Tax/CREB/viral CRE DNA complex.	bind
10494	2	4185	5	11	NULL	NULL	NULL	coactivators	GP		bind					Tax/CREB/viral CRE DNA complex	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_10_3392_s_114	12724399	(B) SREBP-1a binding to the KIX domain of full-length CBP/p300 prevents binding of the coactivators to the Tax/CREB/viral CRE DNA complex.	bind
10495	3	4185	5	11	NULL	NULL	NULL	statement 1	Process		prevent					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_10_3392_s_114	12724399	(B) SREBP-1a binding to the KIX domain of full-length CBP/p300 prevents binding of the coactivators to the Tax/CREB/viral CRE DNA complex.	bind
12920	1	4185	7	11	NULL	NULL	NULL	 SREBP-1a	GP		bind					CBP/p300	GP	full-length	KIX domain		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_10_3392_s_114	12724399	(B) SREBP-1a binding to the KIX domain of full-length CBP/p300 prevents binding of the coactivators to the Tax/CREB/viral CRE DNA complex.	bind
12921	2	4185	7	11	NULL	NULL	NULL	coactivators 	GP		bind					Tax/CREB/viral CRE DNA complex	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_10_3392_s_114	12724399	(B) SREBP-1a binding to the KIX domain of full-length CBP/p300 prevents binding of the coactivators to the Tax/CREB/viral CRE DNA complex.	bind
12922	3	4185	7	11	NULL	NULL	NULL	statement 1	Process		prevents					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_10_3392_s_114	12724399	(B) SREBP-1a binding to the KIX domain of full-length CBP/p300 prevents binding of the coactivators to the Tax/CREB/viral CRE DNA complex.	bind
10496	1	4186	5	11	NULL	NULL	NULL	SspB	GP		bind					ssrA peptide	GP		NKKGRHGAANDENYALAA		NULL		NULL	NULL	NULL	NULL	gw60_chembiol_9_11_1237_s_60	12445774	(B) SspB binding to the NKKGRHGAANDENYALAA ssrA peptide assayed by isothermal titration calorimetry (25 degrees C).	bind
12923	1	4186	7	11	NULL	NULL	NULL	SspB	GP		bind					 ssrA peptide	GP		NKKGRHGAANDENYALAA		NULL		NULL	NULL	NULL	NULL	gw60_chembiol_9_11_1237_s_60	12445774	(B) SspB binding to the NKKGRHGAANDENYALAA ssrA peptide assayed by isothermal titration calorimetry (25 degrees C).	bind
10500	1	4187	5	11	NULL	NULL	NULL	Ste12	GP		bind									UAS2-1	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_216	15485921	(B) Ste12 and Tec1 binding to UAS2-1 is independent of Flo8 and Mss11.	bind
10501	2	4187	5	11	NULL	NULL	NULL	statement 1	Process		is independent of					Flo8	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_216	15485921	(B) Ste12 and Tec1 binding to UAS2-1 is independent of Flo8 and Mss11.	bind
10502	3	4187	5	11	NULL	NULL	NULL	statement 1	Process		is independent of					Mss11	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_216	15485921	(B) Ste12 and Tec1 binding to UAS2-1 is independent of Flo8 and Mss11.	bind
10503	4	4187	5	11	NULL	NULL	NULL	Tec1	GP		bind									UAS2-1	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_216	15485921	(B) Ste12 and Tec1 binding to UAS2-1 is independent of Flo8 and Mss11.	bind
10504	5	4187	5	11	NULL	NULL	NULL	statement 4	Process		is independent of					Flo8	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_216	15485921	(B) Ste12 and Tec1 binding to UAS2-1 is independent of Flo8 and Mss11.	bind
10505	6	4187	5	11	NULL	NULL	NULL	statement 4	Process		is independent of					Mss11	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_216	15485921	(B) Ste12 and Tec1 binding to UAS2-1 is independent of Flo8 and Mss11.	bind
12924	1	4187	7	11	NULL	NULL	NULL	Ste12 	GP		bind									UAS2-1	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_216	15485921	(B) Ste12 and Tec1 binding to UAS2-1 is independent of Flo8 and Mss11.	bind
12925	2	4187	7	11	NULL	NULL	NULL	Tec1	GP		bind									UAS2-1	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_216	15485921	(B) Ste12 and Tec1 binding to UAS2-1 is independent of Flo8 and Mss11.	bind
12926	3	4187	7	11	NULL	NULL	NULL	statement 1	Process		is independent of					Flo8	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_216	15485921	(B) Ste12 and Tec1 binding to UAS2-1 is independent of Flo8 and Mss11.	bind
12927	4	4187	7	11	NULL	NULL	NULL	statement 2	Process		is independent of					Flo8	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_216	15485921	(B) Ste12 and Tec1 binding to UAS2-1 is independent of Flo8 and Mss11.	bind
12928	5	4187	7	11	NULL	NULL	NULL	statement 1	Process		is independent of					Mss11	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_216	15485921	(B) Ste12 and Tec1 binding to UAS2-1 is independent of Flo8 and Mss11.	bind
12929	6	4187	7	11	NULL	NULL	NULL	statement 2	Process		is independent of					Mss11	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9542_s_216	15485921	(B) Ste12 and Tec1 binding to UAS2-1 is independent of Flo8 and Mss11.	bind
10506	1	4191	5	11	NULL	NULL	NULL	NAD+	Chemical		bind					LeuDH	GP				NULL		NULL	NULL	NULL	NULL	gw60_structure_3_7_693_s_188	8591046	(b) Stereo representation of NAD+ bound to LeuDH.	bind
12930	1	4191	7	11	NULL	NULL	NULL	NAD+	Chemical		bind					LeuDH	GP				NULL		NULL	NULL	NULL	NULL	gw60_structure_3_7_693_s_188	8591046	(b) Stereo representation of NAD+ bound to LeuDH.	bind
10507	1	4192	5	11	NULL	NULL	NULL	HP0525	GP		bind					ADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_6_1461_s_64	11163218	(B) Stereo ribbon diagram of the structure of HP0525 bound to ADP and a 9-mer of PEG ( Carson 1997  ).	bind
10508	2	4192	5	11	NULL	NULL	NULL	HP0525	GP		bind					PEG	Chemical	9-mer of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_6_1461_s_64	11163218	(B) Stereo ribbon diagram of the structure of HP0525 bound to ADP and a 9-mer of PEG ( Carson 1997  ).	bind
12931	1	4192	7	11	NULL	NULL	NULL	HP0525	GP		bind					ADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_6_1461_s_64	11163218	(B) Stereo ribbon diagram of the structure of HP0525 bound to ADP and a 9-mer of PEG ( Carson 1997  ).	bind
12932	2	4192	7	11	NULL	NULL	NULL	HP0525	GP		bind					 PEG	Chemical	9-mer of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_6_1461_s_64	11163218	(B) Stereo ribbon diagram of the structure of HP0525 bound to ADP and a 9-mer of PEG ( Carson 1997  ).	bind
10509	1	4193	5	11	NULL	NULL	NULL	compound 1	Chemical		bind					JNK3	GP		ATP binding site of		NULL		NULL	NULL	NULL	NULL	gw60_chembiol_10_8_705_s_55	12954329	(B) Stereo view of compound 1 bound to the ATP binding site of JNK3.	bind
12933	1	4193	7	11	NULL	NULL	NULL	compound 1	Chemical		bind					JNK3	GP		ATP binding site		NULL		NULL	NULL	NULL	NULL	gw60_chembiol_10_8_705_s_55	12954329	(B) Stereo view of compound 1 bound to the ATP binding site of JNK3.	bind
10510	1	4194	5	11	NULL	NULL	NULL	[35] GTP S	Chemical		bind					PM	QuantityOrMeasure	from limbic forebrain			NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_50_7_834_s_217	16448676	(b) Stimulation of [35] GTP S binding to PM from the limbic forebrain by various concentrations of WIN55,212-2.	bind
10511	2	4194	5	11	NULL	NULL	NULL	WIN55,212-2	Chemical		stimulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_50_7_834_s_217	16448676	(b) Stimulation of [35] GTP S binding to PM from the limbic forebrain by various concentrations of WIN55,212-2.	bind
12934	1	4194	7	11	NULL	NULL	NULL	[35] GTP S	Chemical		binds to					PM	QuantityOrMeasure	limbic forebrain			NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_50_7_834_s_217	16448676	(b) Stimulation of [35] GTP S binding to PM from the limbic forebrain by various concentrations of WIN55,212-2.	bind
16309	2	4194	7	11	NULL	NULL	NULL	WIN55,212-2	Chemical		stimulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_50_7_834_s_217	16448676	(b) Stimulation of [35] GTP S binding to PM from the limbic forebrain by various concentrations of WIN55,212-2.	bind
10512	1	4196	5	11	NULL	NULL	NULL	E-cadherin	GP	phosphorylated	bind			region IV		beta-catenin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_105_3_391_s_135	11348595	(B) Structure of  phosphorylated E-cadherin region IV bound to beta-catenin.	bind
12935	1	4196	7	11	NULL	NULL	NULL	 E-cadherin	GP	phosphorylated	bind			region IV		beta-catenin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_105_3_391_s_135	11348595	(B) Structure of  phosphorylated E-cadherin region IV bound to beta-catenin.	bind
10513	1	4197	5	11	NULL	NULL	NULL	Lyn	GP		bind					CD19	GP	phosphorylated	Y513		NULL		NULL	NULL	NULL	NULL	gw60_immunity_13_1_47_s_265	10933394	(B) Subsequently, Lyn binds phosphorylated CD19-Y513 via its SH2 domain and phosphorylates CD19-Y482 through  processive phosphorylation.	bind
10514	2	4197	5	11	NULL	NULL	NULL	statement 1	Process		via					CD19	GP		SH2 domain		NULL		NULL	NULL	NULL	NULL	gw60_immunity_13_1_47_s_265	10933394	(B) Subsequently, Lyn binds phosphorylated CD19-Y513 via its SH2 domain and phosphorylates CD19-Y482 through  processive phosphorylation.	bind
10515	3	4197	5	11	NULL	NULL	NULL	Lyn	GP		phosphorylate					CD19	GP		Y482		NULL		NULL	NULL	NULL	NULL	gw60_immunity_13_1_47_s_265	10933394	(B) Subsequently, Lyn binds phosphorylated CD19-Y513 via its SH2 domain and phosphorylates CD19-Y482 through  processive phosphorylation.	bind
10516	4	4197	5	11	NULL	NULL	NULL	statement 3	Process		occurs through					processive phosphorylation	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_13_1_47_s_265	10933394	(B) Subsequently, Lyn binds phosphorylated CD19-Y513 via its SH2 domain and phosphorylates CD19-Y482 through  processive phosphorylation.	bind
12936	1	4197	7	11	NULL	NULL	NULL	Lyn	GP		binds					CD19	GP	 phosphorylated	Y513 SH2 domain		NULL		NULL	NULL	NULL	NULL	gw60_immunity_13_1_47_s_265	10933394	(B) Subsequently, Lyn binds phosphorylated CD19-Y513 via its SH2 domain and phosphorylates CD19-Y482 through  processive phosphorylation.	bind
12937	2	4197	7	11	NULL	NULL	NULL	statement 1	GP		phosphorylates					CD19	GP		Y482		NULL		NULL	NULL	NULL	NULL	gw60_immunity_13_1_47_s_265	10933394	(B) Subsequently, Lyn binds phosphorylated CD19-Y513 via its SH2 domain and phosphorylates CD19-Y482 through  processive phosphorylation.	bind
12938	3	4197	7	11	NULL	NULL	NULL	statement 1	Process		occurs through					processive phosphorylation	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_13_1_47_s_265	10933394	(B) Subsequently, Lyn binds phosphorylated CD19-Y513 via its SH2 domain and phosphorylates CD19-Y482 through  processive phosphorylation.	bind
10517	1	4200	5	11	NULL	NULL	NULL	Pho81	GP		bind					Pho80-Pho85	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6695_s_247	11533256	(B) Summary of the binding of different Pho81 domains to Pho80-Pho85.	bind
12939	1	4200	7	11	NULL	NULL	NULL	Pho81	GP		binds					Pho80-Pho85	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6695_s_247	11533256	(B) Summary of the binding of different Pho81 domains to Pho80-Pho85.	bind
12458	1	4201	5	11	NULL	NULL	NULL			SUMO- modified	bind			CRD1 domain		HDAC6	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcell_11_4_1043_s_220	12718889	(B) SUMO- modified CRD1 domain binds HDAC6 in vitro.	bind
12940	1	4201	7	11	NULL	NULL	NULL			SUMO- modified	binds			CRD1 domain		HDAC6	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcell_11_4_1043_s_220	12718889	(B) SUMO- modified CRD1 domain binds HDAC6 in vitro.	bind
12459	1	4203	5	11	NULL	NULL	NULL	caspase-7	GP	active	bind					XIAP fragment	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_3_399_s_181	11701129	(B) Superposition  of the active caspase-7 without bound cofactors  (pink), the procaspase-7 zymogen (blue), and the active caspase-7  (green) bound with an XIAP fragment.	bind
12941	1	4203	7	11	NULL	NULL	NULL	caspase-7	GP	active	bind					XIAP fragment	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_3_399_s_181	11701129	(B) Superposition  of the active caspase-7 without bound cofactors  (pink), the procaspase-7 zymogen (blue), and the active caspase-7  (green) bound with an XIAP fragment.	bind
12460	1	4204	5	11	NULL	NULL	NULL	threonyl-tRNA synthetase	GP		bind			C-terminal domain		cognate tRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_1_43_s_71	11172710	(B) Superposition of domain 3 of Pol B with the C-terminal domain of threonyl-tRNA synthetase bound to its cognate tRNA ( Yaremchuk et al. 2000  ; PDB code 1QF6).	bind
12942	1	4204	7	11	NULL	NULL	NULL	threonyl-tRNA synthetase	GP		binds			C-terminal domain		cognate tRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_1_43_s_71	11172710	(B) Superposition of domain 3 of Pol B with the C-terminal domain of threonyl-tRNA synthetase bound to its cognate tRNA ( Yaremchuk et al. 2000  ; PDB code 1QF6).	bind
12461	1	4205	5	11	NULL	NULL	NULL	GL-7-ACA	Chemical		bind					CAD	GP				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_12_1253_s_225	11755403	(B) Superposition of GL-7-ACA bound CAD onto PMSF bound PGA with four catalytic residues  [28]  .	bind
12462	2	4205	5	11	NULL	NULL	NULL	PMSF	Chemical		bind					PGA	GP				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_12_1253_s_225	11755403	(B) Superposition of GL-7-ACA bound CAD onto PMSF bound PGA with four catalytic residues  [28]  .	bind
12943	1	4205	7	11	NULL	NULL	NULL	GL-7-ACA	Chemical		bind					CAD	GP				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_12_1253_s_225	11755403	(B) Superposition of GL-7-ACA bound CAD onto PMSF bound PGA with four catalytic residues  [28]  .	bind
12944	2	4205	7	11	NULL	NULL	NULL	PMSF	Chemical		bind					PGA	GP				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_12_1253_s_225	11755403	(B) Superposition of GL-7-ACA bound CAD onto PMSF bound PGA with four catalytic residues  [28]  .	bind
13447	1	4206	5	11	NULL	NULL	NULL	TS: TS	GP	Escherichia coli	bind					dUMP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_5_445_s_144	11358692	(b) Superposition of seven structures of TS: TS from  Escherichia coli bound to dUMP and either CB3717, BW1843U89 or ZD1694, PcTS bound to dUMP and either CB3717 or BW1843U89 and TS from  Lactobacillus casei bound to A156 or MR29.	bind
43350	2	4206	5	11	NULL	NULL	NULL	TS: TS	GP	Escherichia coli	bind					CB3717	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_5_445_s_144	11358692	(b) Superposition of seven structures of TS: TS from  Escherichia coli bound to dUMP and either CB3717, BW1843U89 or ZD1694, PcTS bound to dUMP and either CB3717 or BW1843U89 and TS from  Lactobacillus casei bound to A156 or MR29.	bind
43351	3	4206	5	11	NULL	NULL	NULL	TS: TS	GP	Escherichia coli	bind					BW1843U89	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_5_445_s_144	11358692	(b) Superposition of seven structures of TS: TS from  Escherichia coli bound to dUMP and either CB3717, BW1843U89 or ZD1694, PcTS bound to dUMP and either CB3717 or BW1843U89 and TS from  Lactobacillus casei bound to A156 or MR29.	bind
43353	4	4206	5	11	NULL	NULL	NULL	TS: TS	GP	Escherichia coli	bind					ZD1694	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_5_445_s_144	11358692	(b) Superposition of seven structures of TS: TS from  Escherichia coli bound to dUMP and either CB3717, BW1843U89 or ZD1694, PcTS bound to dUMP and either CB3717 or BW1843U89 and TS from  Lactobacillus casei bound to A156 or MR29.	bind
43354	5	4206	5	11	NULL	NULL	NULL	PcTS	Organism		bind					dUMP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_5_445_s_144	11358692	(b) Superposition of seven structures of TS: TS from  Escherichia coli bound to dUMP and either CB3717, BW1843U89 or ZD1694, PcTS bound to dUMP and either CB3717 or BW1843U89 and TS from  Lactobacillus casei bound to A156 or MR29.	bind
43355	6	4206	5	11	NULL	NULL	NULL	PcTS	Organism		bind					CB3717	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_5_445_s_144	11358692	(b) Superposition of seven structures of TS: TS from  Escherichia coli bound to dUMP and either CB3717, BW1843U89 or ZD1694, PcTS bound to dUMP and either CB3717 or BW1843U89 and TS from  Lactobacillus casei bound to A156 or MR29.	bind
43357	7	4206	5	11	NULL	NULL	NULL	PcTS	Organism		bind					BW1843U89	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_5_445_s_144	11358692	(b) Superposition of seven structures of TS: TS from  Escherichia coli bound to dUMP and either CB3717, BW1843U89 or ZD1694, PcTS bound to dUMP and either CB3717 or BW1843U89 and TS from  Lactobacillus casei bound to A156 or MR29.	bind
43358	8	4206	5	11	NULL	NULL	NULL	TS	Organism	Lactobacillus casei	bind								A156		NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_5_445_s_144	11358692	(b) Superposition of seven structures of TS: TS from  Escherichia coli bound to dUMP and either CB3717, BW1843U89 or ZD1694, PcTS bound to dUMP and either CB3717 or BW1843U89 and TS from  Lactobacillus casei bound to A156 or MR29.	bind
43360	9	4206	5	11	NULL	NULL	NULL	TS	Organism	Lactobacillus casei	bind					MR29	GP				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_5_445_s_144	11358692	(b) Superposition of seven structures of TS: TS from  Escherichia coli bound to dUMP and either CB3717, BW1843U89 or ZD1694, PcTS bound to dUMP and either CB3717 or BW1843U89 and TS from  Lactobacillus casei bound to A156 or MR29.	bind
12945	1	4206	7	11	NULL	NULL	NULL	TS: TS	Organism	Escherichia coli	bind					dUMP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_5_445_s_144	11358692	(b) Superposition of seven structures of TS: TS from  Escherichia coli bound to dUMP and either CB3717, BW1843U89 or ZD1694, PcTS bound to dUMP and either CB3717 or BW1843U89 and TS from  Lactobacillus casei bound to A156 or MR29.	bind
12946	2	4206	7	11	NULL	NULL	NULL	TS: TS 	GP	Escherichia coli	bind					CB3717	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_5_445_s_144	11358692	(b) Superposition of seven structures of TS: TS from  Escherichia coli bound to dUMP and either CB3717, BW1843U89 or ZD1694, PcTS bound to dUMP and either CB3717 or BW1843U89 and TS from  Lactobacillus casei bound to A156 or MR29.	bind
12947	3	4206	7	11	NULL	NULL	NULL	TS: TS	GP	Escherichia coli	bind					BW1843U89	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_5_445_s_144	11358692	(b) Superposition of seven structures of TS: TS from  Escherichia coli bound to dUMP and either CB3717, BW1843U89 or ZD1694, PcTS bound to dUMP and either CB3717 or BW1843U89 and TS from  Lactobacillus casei bound to A156 or MR29.	bind
12948	4	4206	7	11	NULL	NULL	NULL	TS: TS	GP	Escherichia coli 	bind					ZD1694	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_5_445_s_144	11358692	(b) Superposition of seven structures of TS: TS from  Escherichia coli bound to dUMP and either CB3717, BW1843U89 or ZD1694, PcTS bound to dUMP and either CB3717 or BW1843U89 and TS from  Lactobacillus casei bound to A156 or MR29.	bind
12949	5	4206	7	11	NULL	NULL	NULL	PcTS	Organism		bind					dUMP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_5_445_s_144	11358692	(b) Superposition of seven structures of TS: TS from  Escherichia coli bound to dUMP and either CB3717, BW1843U89 or ZD1694, PcTS bound to dUMP and either CB3717 or BW1843U89 and TS from  Lactobacillus casei bound to A156 or MR29.	bind
12950	6	4206	7	11	NULL	NULL	NULL	PcTS	Organism		bind					CB3717	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_5_445_s_144	11358692	(b) Superposition of seven structures of TS: TS from  Escherichia coli bound to dUMP and either CB3717, BW1843U89 or ZD1694, PcTS bound to dUMP and either CB3717 or BW1843U89 and TS from  Lactobacillus casei bound to A156 or MR29.	bind
12951	7	4206	7	11	NULL	NULL	NULL	PcTS	Organism		bind					BW1843U89 	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_5_445_s_144	11358692	(b) Superposition of seven structures of TS: TS from  Escherichia coli bound to dUMP and either CB3717, BW1843U89 or ZD1694, PcTS bound to dUMP and either CB3717 or BW1843U89 and TS from  Lactobacillus casei bound to A156 or MR29.	bind
12952	8	4206	7	11	NULL	NULL	NULL	TS	GP	Lactobacillus casei	bind								A156		NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_5_445_s_144	11358692	(b) Superposition of seven structures of TS: TS from  Escherichia coli bound to dUMP and either CB3717, BW1843U89 or ZD1694, PcTS bound to dUMP and either CB3717 or BW1843U89 and TS from  Lactobacillus casei bound to A156 or MR29.	bind
12953	10	4206	7	11	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_5_445_s_144	11358692	(b) Superposition of seven structures of TS: TS from  Escherichia coli bound to dUMP and either CB3717, BW1843U89 or ZD1694, PcTS bound to dUMP and either CB3717 or BW1843U89 and TS from  Lactobacillus casei bound to A156 or MR29.	bind
12954	11	4206	7	11	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_5_445_s_144	11358692	(b) Superposition of seven structures of TS: TS from  Escherichia coli bound to dUMP and either CB3717, BW1843U89 or ZD1694, PcTS bound to dUMP and either CB3717 or BW1843U89 and TS from  Lactobacillus casei bound to A156 or MR29.	bind
12955	9	4206	7	11	NULL	NULL	NULL	TS	GP	Lactobacillus casei	bind					MR29	GP				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_5_445_s_144	11358692	(b) Superposition of seven structures of TS: TS from  Escherichia coli bound to dUMP and either CB3717, BW1843U89 or ZD1694, PcTS bound to dUMP and either CB3717 or BW1843U89 and TS from  Lactobacillus casei bound to A156 or MR29.	bind
54321	12	4206	7	11	NULL	NULL	NULL	statement 6	Process		is an alternative to					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_5_445_s_144	11358692	(b) Superposition of seven structures of TS: TS from  Escherichia coli bound to dUMP and either CB3717, BW1843U89 or ZD1694, PcTS bound to dUMP and either CB3717 or BW1843U89 and TS from  Lactobacillus casei bound to A156 or MR29.	bind
54322	13	4206	7	11	NULL	NULL	NULL	statement 8	Process		is an alternative to					statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_5_445_s_144	11358692	(b) Superposition of seven structures of TS: TS from  Escherichia coli bound to dUMP and either CB3717, BW1843U89 or ZD1694, PcTS bound to dUMP and either CB3717 or BW1843U89 and TS from  Lactobacillus casei bound to A156 or MR29.	bind
12463	1	4207	5	11	NULL	NULL	NULL	EPA	Chemical		bind					PPAR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_3_397_s_151	10198642	(b) Superposition of the structures of GW2433 and EPA bound to PPAR .	bind
16472	2	4207	5	11	NULL	NULL	NULL	GW2433	Chemical		bind					PPAR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_3_397_s_151	10198642	(b) Superposition of the structures of GW2433 and EPA bound to PPAR .	bind
12956	1	4207	7	11	NULL	NULL	NULL	GW2433	Chemical		bind					PPAR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_3_397_s_151	10198642	(b) Superposition of the structures of GW2433 and EPA bound to PPAR .	bind
12957	2	4207	7	11	NULL	NULL	NULL	EPA	Chemical		bind					PPAR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_3_397_s_151	10198642	(b) Superposition of the structures of GW2433 and EPA bound to PPAR .	bind
12464	1	4208	5	11	NULL	NULL	NULL	caspase-7	GP	active	bind					XIAP fragment	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_3_399_s_47	11701129	(B) Superposition of the unprocessed procaspase-7 zymogen  (blue) with the active caspase-7 (green) bound with an  XIAP fragment.	bind
12958	1	4208	7	11	NULL	NULL	NULL	caspase-7	GP	active	bind					 XIAP fragment	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_3_399_s_47	11701129	(B) Superposition of the unprocessed procaspase-7 zymogen  (blue) with the active caspase-7 (green) bound with an  XIAP fragment.	bind
12465	1	4210	5	11	NULL	NULL	NULL	CBP20	GP	TAPmyc-tagged	bind					SL RNA	NucleicAcid	32P-labeled			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2216_s_109	15743819	(B) Supershift analysis of CBP20 binding to the SL RNA. 32P-labeled SL RNA (lane 1) was incubated with TAPmyc-tagged CBP20, partially purified by the TAP method, in the absence of antibodies  (lane 2) or in the presence of anti-myc (lane 3) and anti-HA (lane 4) antibodies.	bind
12959	1	4210	7	11	NULL	NULL	NULL	CBP20	GP	TAPmyc-tagged	bind					SL RNA	NucleicAcid	32P-labeled			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2216_s_109	15743819	(B) Supershift analysis of CBP20 binding to the SL RNA. 32P-labeled SL RNA (lane 1) was incubated with TAPmyc-tagged CBP20, partially purified by the TAP method, in the absence of antibodies  (lane 2) or in the presence of anti-myc (lane 3) and anti-HA (lane 4) antibodies.	bind
12466	1	4211	5	11	NULL	NULL	NULL	AP-1	GP		bind		specifically			c-Jun	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainres_872_1_282_s_81	10924710	(B) Supershift of AP-1 binding by specific antibodies against c-Jun and ATF-2.	bind
12467	2	4211	5	11	NULL	NULL	NULL	AP-1	GP		bind		specifically			ATF-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainres_872_1_282_s_81	10924710	(B) Supershift of AP-1 binding by specific antibodies against c-Jun and ATF-2.	bind
12960	1	4211	7	11	NULL	NULL	NULL	AP-1	GP		bind		specifically			c-Jun antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainres_872_1_282_s_81	10924710	(B) Supershift of AP-1 binding by specific antibodies against c-Jun and ATF-2.	bind
12961	2	4211	7	11	NULL	NULL	NULL	AP-1	GP		bind		specifically			ATF-2 antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainres_872_1_282_s_81	10924710	(B) Supershift of AP-1 binding by specific antibodies against c-Jun and ATF-2.	bind
12523	1	4212	5	11	NULL	NULL	NULL	CUS2 alleles	GP		supress									G53A	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5000_s_145	9710584	(B) Suppression of G53A and C62U by different  CUS2 alleles.	bind
12525	2	4212	5	11	NULL	NULL	NULL	CUS2 alleles	GP		supress									C62U	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5000_s_145	9710584	(B) Suppression of G53A and C62U by different  CUS2 alleles.	bind
12962	1	4212	7	11	NULL	NULL	NULL	CUS2 alleles	GP		suppress									G53A 	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5000_s_145	9710584	(B) Suppression of G53A and C62U by different  CUS2 alleles.	bind
12963	2	4212	7	11	NULL	NULL	NULL	CUS2 alleles	GP		suppress									C62U	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5000_s_145	9710584	(B) Suppression of G53A and C62U by different  CUS2 alleles.	bind
12527	1	4213	5	11	NULL	NULL	NULL	SWI/SNF	GP		bind					HO	GP			URS1	NULL	during the cell cycle	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4095_s_143	16705163	(B) SWI/SNF binding to  HO URS1 and URS2 during the cell cycle.	bind
12528	2	4213	5	11	NULL	NULL	NULL	SWI/SNF	GP		bind					HO	GP			URS2	NULL	during the cell cycle	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4095_s_143	16705163	(B) SWI/SNF binding to  HO URS1 and URS2 during the cell cycle.	bind
12964	1	4213	7	11	NULL	NULL	NULL	SWI/SNF	GP		bind					HO	GP			URS1	NULL	during cell cycle	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4095_s_143	16705163	(B) SWI/SNF binding to  HO URS1 and URS2 during the cell cycle.	bind
12965	2	4213	7	11	NULL	NULL	NULL	SWI/SNF	GP		bind					HO	GP			URS2	NULL	during cell cycle	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4095_s_143	16705163	(B) SWI/SNF binding to  HO URS1 and URS2 during the cell cycle.	bind
12540	1	4214	5	11	NULL	NULL	NULL	PGL-1	GP	native	bind					Schwann cell-DRG neuron co-cultures	Cell				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_3_511_s_106	11081637	(B) Synthetic trisaccharides inhibit native PGL-1 binding  to Schwann cell-DRG neuron co-cultures.	bind
12542	2	4214	5	11	NULL	NULL	NULL	trisaccharides	Chemical	synthetic	inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_3_511_s_106	11081637	(B) Synthetic trisaccharides inhibit native PGL-1 binding  to Schwann cell-DRG neuron co-cultures.	bind
12966	1	4214	7	11	NULL	NULL	NULL	PGL-1	GP	native	binds					Schwann cell-DRG neuron co-culture	Cell				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_3_511_s_106	11081637	(B) Synthetic trisaccharides inhibit native PGL-1 binding  to Schwann cell-DRG neuron co-cultures.	bind
12967	2	4214	7	11	NULL	NULL	NULL	trisaccharides	Chemical	synthetic	inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_3_511_s_106	11081637	(B) Synthetic trisaccharides inhibit native PGL-1 binding  to Schwann cell-DRG neuron co-cultures.	bind
12545	1	4215	5	11	NULL	NULL	NULL	telomeric DNA	NucleicAcid		bind					xTRF chimeric proteins	GP				NULL	in Xenopus egg extracts	NULL	NULL	NULL	NULL	gw70_embo_25_3_575_s_139	16424898	(B) Telomeric  DNA binding of chimeric xTRF proteins in  Xenopus egg extracts.	bind
12968	1	4215	7	11	NULL	NULL	NULL	chimeric xTRF protein	GP		bind					Telomeric DNA	NucleicAcid				NULL	Xenopus egg extracts	NULL	NULL	NULL	NULL	gw70_embo_25_3_575_s_139	16424898	(B) Telomeric  DNA binding of chimeric xTRF proteins in  Xenopus egg extracts.	bind
12549	1	4216	5	11	NULL	NULL	NULL	FLO11	GP		bind				FRE of promoter	Ste12p protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_1_161_s_212	9436998	(B) The   FLO11 promoter region contains a filamentous response element (FRE), a site for the cooperative binding of the proteins Ste12p and Tec1p which transcriptionally activate genes during the filamentous response (Madhani and Fink, 1997  ).	bind
12550	2	4216	5	11	NULL	NULL	NULL	FRE	GP		is					filamentous response element	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_1_161_s_212	9436998	(B) The   FLO11 promoter region contains a filamentous response element (FRE), a site for the cooperative binding of the proteins Ste12p and Tec1p which transcriptionally activate genes during the filamentous response (Madhani and Fink, 1997  ).	bind
12551	3	4216	5	11	NULL	NULL	NULL	FLO11	GP		bind				FRE of promoter	Tec1p  protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_1_161_s_212	9436998	(B) The   FLO11 promoter region contains a filamentous response element (FRE), a site for the cooperative binding of the proteins Ste12p and Tec1p which transcriptionally activate genes during the filamentous response (Madhani and Fink, 1997  ).	bind
54278	4	4216	5	11	NULL	NULL	NULL	statement 1	Process		occurs in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_1_161_s_212	9436998	(B) The   FLO11 promoter region contains a filamentous response element (FRE), a site for the cooperative binding of the proteins Ste12p and Tec1p which transcriptionally activate genes during the filamentous response (Madhani and Fink, 1997  ).	bind
12969	1	4216	7	11	NULL	NULL	NULL	Ste12p	GP		bind					FLO11	GP			FRE of promoter	NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_1_161_s_212	9436998	(B) The   FLO11 promoter region contains a filamentous response element (FRE), a site for the cooperative binding of the proteins Ste12p and Tec1p which transcriptionally activate genes during the filamentous response (Madhani and Fink, 1997  ).	bind
12970	2	4216	7	11	NULL	NULL	NULL	Tec1p	GP		bind					FLO11	GP			FRE of promoter	NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_1_161_s_212	9436998	(B) The   FLO11 promoter region contains a filamentous response element (FRE), a site for the cooperative binding of the proteins Ste12p and Tec1p which transcriptionally activate genes during the filamentous response (Madhani and Fink, 1997  ).	bind
12972	4	4216	7	11	NULL	NULL	NULL	FRE	GP		is					filamentous response element	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_1_161_s_212	9436998	(B) The   FLO11 promoter region contains a filamentous response element (FRE), a site for the cooperative binding of the proteins Ste12p and Tec1p which transcriptionally activate genes during the filamentous response (Madhani and Fink, 1997  ).	bind
54279	3	4216	7	11	NULL	NULL	NULL	statement 1	Process		occurs in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_1_161_s_212	9436998	(B) The   FLO11 promoter region contains a filamentous response element (FRE), a site for the cooperative binding of the proteins Ste12p and Tec1p which transcriptionally activate genes during the filamentous response (Madhani and Fink, 1997  ).	bind
12557	1	4217	5	11	NULL	NULL	NULL	eIF5	GP		bind					NIP1	GP		NTD		NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9437_s_254	15485912	(B) The  NIP1-Box2 mutation diminishes binding of eIF5 and eIF2 to the NIP1-NTD in vivo.	bind
12559	2	4217	5	11	NULL	NULL	NULL	eIF2	GP		bind					NIP1	GP		NTD		NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9437_s_254	15485912	(B) The  NIP1-Box2 mutation diminishes binding of eIF5 and eIF2 to the NIP1-NTD in vivo.	bind
12560	3	4217	5	11	NULL	NULL	NULL	NIP1	GP	mutant	diminishes			Box2		statement 1	Process				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9437_s_254	15485912	(B) The  NIP1-Box2 mutation diminishes binding of eIF5 and eIF2 to the NIP1-NTD in vivo.	bind
12562	4	4217	5	11	NULL	NULL	NULL	NIP1	GP	mutant	diminishes			Box2		statement 2	Process				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9437_s_254	15485912	(B) The  NIP1-Box2 mutation diminishes binding of eIF5 and eIF2 to the NIP1-NTD in vivo.	bind
12975	1	4217	7	11	NULL	NULL	NULL	eIF5	GP		bind					NIP1	GP		NTD		NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9437_s_254	15485912	(B) The  NIP1-Box2 mutation diminishes binding of eIF5 and eIF2 to the NIP1-NTD in vivo.	bind
12976	2	4217	7	11	NULL	NULL	NULL	eIF2	GP		bind					NIP1	GP		NTD		NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9437_s_254	15485912	(B) The  NIP1-Box2 mutation diminishes binding of eIF5 and eIF2 to the NIP1-NTD in vivo.	bind
12977	3	4217	7	11	NULL	NULL	NULL	NIP1	GP	mutation of	diminishes			Box2		statement 1	Process				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9437_s_254	15485912	(B) The  NIP1-Box2 mutation diminishes binding of eIF5 and eIF2 to the NIP1-NTD in vivo.	bind
12978	4	4217	7	11	NULL	NULL	NULL	NIP1	GP	mutation of	diminishes			Box2		statement 2	Process				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9437_s_254	15485912	(B) The  NIP1-Box2 mutation diminishes binding of eIF5 and eIF2 to the NIP1-NTD in vivo.	bind
12568	1	4218	5	11	NULL	NULL	NULL	41 kDa proteins	GP		bind					NF 3-GST	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_4_3_419_s_78	12636922	(B) The 41 and 39 kDa proteins bound by NF 3-GST are identical to human TAF1.	bind
12570	2	4218	5	11	NULL	NULL	NULL	statement 1	GP		identical to					TAF1	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_devcell_4_3_419_s_78	12636922	(B) The 41 and 39 kDa proteins bound by NF 3-GST are identical to human TAF1.	bind
12571	3	4218	5	11	NULL	NULL	NULL	39 kDa proteins	GP		bind					NF 3-GST	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_4_3_419_s_78	12636922	(B) The 41 and 39 kDa proteins bound by NF 3-GST are identical to human TAF1.	bind
12576	4	4218	5	11	NULL	NULL	NULL	statement 3	GP		identical to					TAF1	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_devcell_4_3_419_s_78	12636922	(B) The 41 and 39 kDa proteins bound by NF 3-GST are identical to human TAF1.	bind
12979	1	4218	7	11	NULL	NULL	NULL	NF 3-GST	GP		bind					41 kDa protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_4_3_419_s_78	12636922	(B) The 41 and 39 kDa proteins bound by NF 3-GST are identical to human TAF1.	bind
12980	2	4218	7	11	NULL	NULL	NULL	NF3-GST	GP		bind					39 kDa protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_4_3_419_s_78	12636922	(B) The 41 and 39 kDa proteins bound by NF 3-GST are identical to human TAF1.	bind
12981	3	4218	7	11	NULL	NULL	NULL	41kDa protein	GP		is identical to					TAF1	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_devcell_4_3_419_s_78	12636922	(B) The 41 and 39 kDa proteins bound by NF 3-GST are identical to human TAF1.	bind
12580	1	4220	5	11	NULL	NULL	NULL	C3	GP		bind					yeast cells	Organism				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_74_7_4310_s_224	16790805	(B) The amount  of C3 binding to yeast cells in the presence of each test antibody was determined  by flow cytometry.	bind
12983	1	4220	7	11	NULL	NULL	NULL	C3	GP		bind					yeast cells	Organism				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_74_7_4310_s_224	16790805	(B) The amount  of C3 binding to yeast cells in the presence of each test antibody was determined  by flow cytometry.	bind
12582	1	4221	5	11	NULL	NULL	NULL	FKBP12	GP		bind					RyR1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_160_6_919_s_106	12629052	(B) The amount of FKBP12 bound to  RyR1 was assessed by coimmunoprecipitation followed by immunoblotting.	bind
12984	1	4221	7	11	NULL	NULL	NULL	FKBP12	GP		bind					RyR1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_160_6_919_s_106	12629052	(B) The amount of FKBP12 bound to  RyR1 was assessed by coimmunoprecipitation followed by immunoblotting.	bind
12583	1	4223	5	11	NULL	NULL	NULL	Cdc68	GP		bind					Nhp6a	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_10_3491_s_263	11313475	(B) The assemblage of Cdc68 and Pob3-Nhp6a protein binds Nhp6a.	bind
12584	2	4223	5	11	NULL	NULL	NULL	Pob3-Nhp6a protein	GP		bind					Nhp6a	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_10_3491_s_263	11313475	(B) The assemblage of Cdc68 and Pob3-Nhp6a protein binds Nhp6a.	bind
12982	4	4223	7	11	NULL	NULL	NULL	39 kDa protein	GP		is identical to					TAF1	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_10_3491_s_263	11313475	(B) The assemblage of Cdc68 and Pob3-Nhp6a protein binds Nhp6a.	bind
12985	1	4223	7	11	NULL	NULL	NULL	Cdc68	GP		bind					Nhp6a	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_10_3491_s_263	11313475	(B) The assemblage of Cdc68 and Pob3-Nhp6a protein binds Nhp6a.	bind
12986	2	4223	7	11	NULL	NULL	NULL	Pob3-Nhp6a	GP		bind					Nhp6a	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_10_3491_s_263	11313475	(B) The assemblage of Cdc68 and Pob3-Nhp6a protein binds Nhp6a.	bind
12585	1	4225	5	11	NULL	NULL	NULL	HDAC1	GP		bind					AR	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8563_s_163	14612401	(B) The binding of HDAC1 to the AR is shown as percent binding for multiple  separate transfections.	bind
12987	1	4225	7	11	NULL	NULL	NULL	HDAC1	GP		bind					AR	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8563_s_163	14612401	(B) The binding of HDAC1 to the AR is shown as percent binding for multiple  separate transfections.	bind
12586	1	4226	5	11	NULL	NULL	NULL	Hha	GP		bind					DNA	NucleicAcid	labeled		hilA promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_22_6620_s_262	11673432	(B) The binding of Hha to labeled  hilA promoter DNA was competed with unlabeled  hilA promoter DNA.	bind
12587	2	4226	5	11	NULL	NULL	NULL	Hha	GP		bind					DNA	NucleicAcid	unlabeled		hilA promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_22_6620_s_262	11673432	(B) The binding of Hha to labeled  hilA promoter DNA was competed with unlabeled  hilA promoter DNA.	bind
12588	3	4226	5	11	NULL	NULL	NULL	statement 1	Process		compete with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_22_6620_s_262	11673432	(B) The binding of Hha to labeled  hilA promoter DNA was competed with unlabeled  hilA promoter DNA.	bind
12988	1	4226	7	11	NULL	NULL	NULL	Hha	GP		bind					hilA DNA	NucleicAcid	labeled		promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_22_6620_s_262	11673432	(B) The binding of Hha to labeled  hilA promoter DNA was competed with unlabeled  hilA promoter DNA.	bind
12989	2	4226	7	11	NULL	NULL	NULL	Hha	GP		bind					hilA DNA	NucleicAcid	unlabeled		promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_22_6620_s_262	11673432	(B) The binding of Hha to labeled  hilA promoter DNA was competed with unlabeled  hilA promoter DNA.	bind
12990	3	4226	7	11	NULL	NULL	NULL	statement 1	Process		compete with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_22_6620_s_262	11673432	(B) The binding of Hha to labeled  hilA promoter DNA was competed with unlabeled  hilA promoter DNA.	bind
12604	1	4227	5	11	NULL	NULL	NULL	Munc18c	GP		bind					Snc2p-PrA	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_927_s_80	16769821	(B) The binding of Munc18c to Snc2p-PrA and GST-tagged syntaxin 4 (Sx4) was  assessed.	bind
12605	2	4227	5	11	NULL	NULL	NULL	Munc18c	GP		bind					GST-tagged syntaxin 4	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_927_s_80	16769821	(B) The binding of Munc18c to Snc2p-PrA and GST-tagged syntaxin 4 (Sx4) was  assessed.	bind
16471	3	4227	5	11	NULL	NULL	NULL	syntaxin 4	GP		is					Sx4	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_927_s_80	16769821	(B) The binding of Munc18c to Snc2p-PrA and GST-tagged syntaxin 4 (Sx4) was  assessed.	bind
12991	1	4227	7	11	NULL	NULL	NULL	Munc18c	GP		bind					Snc2p-PrA	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_927_s_80	16769821	(B) The binding of Munc18c to Snc2p-PrA and GST-tagged syntaxin 4 (Sx4) was  assessed.	bind
12992	2	4227	7	11	NULL	NULL	NULL	Munc18c	GP		bind					syntaxin 4	GP	GST-tagged			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_927_s_80	16769821	(B) The binding of Munc18c to Snc2p-PrA and GST-tagged syntaxin 4 (Sx4) was  assessed.	bind
12993	3	4227	7	11	NULL	NULL	NULL	syntaxin 4	GP		is					Sx4	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_6_927_s_80	16769821	(B) The binding of Munc18c to Snc2p-PrA and GST-tagged syntaxin 4 (Sx4) was  assessed.	bind
12994	1	4228	7	11	NULL	NULL	NULL	PPAR	GP		bind					Site I 	NucleicAcid	truncated derivative of			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1583_2_229_s_113	12117567	(B) The binding of PPAR , LXR  and RXR  to a truncated derivative of the Site I comprising the 5' half site of the LXRE plus the next six consecutive nucleotides (see  Table 1 for sequence).	bind
12995	2	4228	7	11	NULL	NULL	NULL	PPAR	GP		bind					statement 1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1583_2_229_s_113	12117567	(B) The binding of PPAR , LXR  and RXR  to a truncated derivative of the Site I comprising the 5' half site of the LXRE plus the next six consecutive nucleotides (see  Table 1 for sequence).	bind
12996	3	4228	7	11	NULL	NULL	NULL	LXR	GP		bind					statement 1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1583_2_229_s_113	12117567	(B) The binding of PPAR , LXR  and RXR  to a truncated derivative of the Site I comprising the 5' half site of the LXRE plus the next six consecutive nucleotides (see  Table 1 for sequence).	bind
12997	1	4228	7	11	NULL	NULL	NULL	Site I	NucleicAcid	truncated derivative of	comprises of									5' half site of the LXRE plus the next six consecutive nucleotides 	NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1583_2_229_s_113	12117567	(B) The binding of PPAR , LXR  and RXR  to a truncated derivative of the Site I comprising the 5' half site of the LXRE plus the next six consecutive nucleotides (see  Table 1 for sequence).	bind
54264	4	4228	7	11	NULL	NULL	NULL	RXR	GP		bind					statement 1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1583_2_229_s_113	12117567	(B) The binding of PPAR , LXR  and RXR  to a truncated derivative of the Site I comprising the 5' half site of the LXRE plus the next six consecutive nucleotides (see  Table 1 for sequence).	bind
12615	1	4229	5	11	NULL	NULL	NULL	TRAF6	GP		bind					CD40	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9806_s_237	16260598	(B) The binding of TRAF6 to CD40 mediates NF-kappaB signaling in TRAF2-deficient cells.	bind
12616	2	4229	5	11	NULL	NULL	NULL	statement 1	Process		mediate					NF-kappaB	GP	signaling of			NULL	in TRAF2-deficient cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9806_s_237	16260598	(B) The binding of TRAF6 to CD40 mediates NF-kappaB signaling in TRAF2-deficient cells.	bind
12998	1	4229	7	11	NULL	NULL	NULL	TRAF6	GP		bind					CD40	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9806_s_237	16260598	(B) The binding of TRAF6 to CD40 mediates NF-kappaB signaling in TRAF2-deficient cells.	bind
12999	2	4229	7	11	NULL	NULL	NULL	statement 1	Process		mediates					NF-kappaB	GP	signaling of			NULL	TRAF2-deficient cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9806_s_237	16260598	(B) The binding of TRAF6 to CD40 mediates NF-kappaB signaling in TRAF2-deficient cells.	bind
12617	1	4230	5	11	NULL	NULL	NULL	CTCF	GP		bind			C terminus		CTCF	GP		11 ZF domain		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_8_3497_s_98	15060168	(B) The C terminus of CTCF binds to the 11 ZF domain of CTCF.	bind
13000	1	4230	7	11	NULL	NULL	NULL	CTCF	GP		bind			C terminus		CTCF	GP		11 ZF domain		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_8_3497_s_98	15060168	(B) The C terminus of CTCF binds to the 11 ZF domain of CTCF.	bind
12618	1	4231	5	11	NULL	NULL	NULL	MIBP1	GP		bind			C-terminal zinc finger		SSTR-2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3736_s_118	10207097	(B) The C-terminal MIBP1 zinc finger binds to the SSTR-2 promoter.	bind
13024	1	4231	7	11	NULL	NULL	NULL	MIBP1	GP		binds to			C-terminal zinc finger		SSTR-2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3736_s_118	10207097	(B) The C-terminal MIBP1 zinc finger binds to the SSTR-2 promoter.	bind
12619	1	4233	5	11	NULL	NULL	NULL	CDC25A	GP		bind			carboxyl terminus		ASK1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_14_4818_s_228	11416155	(B) The carboxyl terminus of CDC25A binds to ASK1 in vitro.	bind
13025	1	4233	7	11	NULL	NULL	NULL	CDC25A	GP		binds			carboxyl terminus		ASK1 	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_14_4818_s_228	11416155	(B) The carboxyl terminus of CDC25A binds to ASK1 in vitro.	bind
13452	1	4234	5	11	NULL	NULL	NULL	NF-E2	GP		bind					HS2 core region	GP	of the transfected muLCR			NULL	in stably transfected MEL cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_9_3083_s_203	11287613	(B) The CCAAT box mutation does not affect the binding of NF-E2 to the HS2 core region of the transfected muLCR in stably transfected MEL cells.	bind
13453	2	4234	5	11	NULL	NULL	NULL			mutant	does not affect				CCAAT box	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_9_3083_s_203	11287613	(B) The CCAAT box mutation does not affect the binding of NF-E2 to the HS2 core region of the transfected muLCR in stably transfected MEL cells.	bind
13026	1	4234	7	11	NULL	NULL	NULL	NF-E2	GP		bind					HS2 core region	GP	transfected muLCR			NULL	transfected MEL cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_9_3083_s_203	11287613	(B) The CCAAT box mutation does not affect the binding of NF-E2 to the HS2 core region of the transfected muLCR in stably transfected MEL cells.	bind
13027	2	4234	7	11	NULL	NULL	NULL			mutation of	does not affect				CCAAT box 	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_9_3083_s_203	11287613	(B) The CCAAT box mutation does not affect the binding of NF-E2 to the HS2 core region of the transfected muLCR in stably transfected MEL cells.	bind
12621	1	4235	5	11	NULL	NULL	NULL	co-activator	GP		bind					Notch 1	GP		IC		NULL		NULL	NULL	NULL	NULL	gw60_mechdev_104_1_3_s_378	11404076	(B) The co-activator (dotted) binds to both Notch 1 IC and Notch 3 IC, but is not sufficient for activation.	bind
12623	2	4235	5	11	NULL	NULL	NULL	co-activator	GP		bind					Notch 3	GP		IC		NULL		NULL	NULL	NULL	NULL	gw60_mechdev_104_1_3_s_378	11404076	(B) The co-activator (dotted) binds to both Notch 1 IC and Notch 3 IC, but is not sufficient for activation.	bind
12624	3	4235	5	11	NULL	NULL	NULL	co-activator	GP		is not sufficient for					activation	Process				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_104_1_3_s_378	11404076	(B) The co-activator (dotted) binds to both Notch 1 IC and Notch 3 IC, but is not sufficient for activation.	bind
13028	1	4235	7	11	NULL	NULL	NULL	co-activator	GP		binds					Notch 1	GP		 IC		NULL		NULL	NULL	NULL	NULL	gw60_mechdev_104_1_3_s_378	11404076	(B) The co-activator (dotted) binds to both Notch 1 IC and Notch 3 IC, but is not sufficient for activation.	bind
13029	2	4235	7	11	NULL	NULL	NULL	co-activator	GP		binds					Notch 3	GP		IC		NULL		NULL	NULL	NULL	NULL	gw60_mechdev_104_1_3_s_378	11404076	(B) The co-activator (dotted) binds to both Notch 1 IC and Notch 3 IC, but is not sufficient for activation.	bind
16310	3	4235	7	11	NULL	NULL	NULL	co-activator	GP		is not sufficient for					activation	Process				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_104_1_3_s_378	11404076	(B) The co-activator (dotted) binds to both Notch 1 IC and Notch 3 IC, but is not sufficient for activation.	bind
12626	1	4236	5	11	NULL	NULL	NULL	E7	Organism	mutant	does not bind			deltaDLYC		Rb	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_378_s_182	9418885	(B) The control for E7 expression was the same expression vector into which a mutant E7 (deltaDLYC) unable to bind Rb was cloned ( 23).	bind
13034	1	4236	7	11	NULL	NULL	NULL	E7	Organism	mutant	does not bind			deltaDLYC		Rb	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_378_s_182	9418885	(B) The control for E7 expression was the same expression vector into which a mutant E7 (deltaDLYC) unable to bind Rb was cloned ( 23).	bind
12628	1	4237	5	11	NULL	NULL	NULL	3H-RTX	Chemical		bind							mutant	S512C		NULL		NULL	NULL	NULL	NULL	gw60_cell_108_3_421_s_171	11853675	(B) The cysteine-reactive reagent MTSET reversibly inhibits 3H-RTX binding to S512C mutant.	bind
12630	2	4237	5	11	NULL	NULL	NULL	MTSET	Chemical		inhibit		reversibly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_108_3_421_s_171	11853675	(B) The cysteine-reactive reagent MTSET reversibly inhibits 3H-RTX binding to S512C mutant.	bind
44432	3	4237	5	11	NULL	NULL	NULL	MTSET	Chemical		is a type of					cysteine-reactive reagent	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_108_3_421_s_171	11853675	(B) The cysteine-reactive reagent MTSET reversibly inhibits 3H-RTX binding to S512C mutant.	bind
13035	1	4237	7	11	NULL	NULL	NULL	3H-RTX	Chemical		binds							mutant	S512C		NULL		NULL	NULL	NULL	NULL	gw60_cell_108_3_421_s_171	11853675	(B) The cysteine-reactive reagent MTSET reversibly inhibits 3H-RTX binding to S512C mutant.	bind
13037	2	4237	7	11	NULL	NULL	NULL	MTSET	Chemical		inhibits		reversibly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_108_3_421_s_171	11853675	(B) The cysteine-reactive reagent MTSET reversibly inhibits 3H-RTX binding to S512C mutant.	bind
44409	3	4237	7	11	NULL	NULL	NULL	MTSET	Chemical		is a type of					cysteine-reactive reagent	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_108_3_421_s_171	11853675	(B) The cysteine-reactive reagent MTSET reversibly inhibits 3H-RTX binding to S512C mutant.	bind
12632	1	4240	5	11	NULL	NULL	NULL	YPT1	GP	wild-type	bind					DSS4	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7444_s_142	9819430	(B) The dominant interfering YPT1-N22 protein binds DSS4 under conditions where the interaction of wild-type YPT1 and DSS4 is disrupted.	bind
12633	2	4240	5	11	NULL	NULL	NULL	YPT1 protein	GP	dominant interfering	bind			N22		DSS4	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7444_s_142	9819430	(B) The dominant interfering YPT1-N22 protein binds DSS4 under conditions where the interaction of wild-type YPT1 and DSS4 is disrupted.	bind
12634	3	4240	5	11	NULL	NULL	NULL	statement 2	Process		occurs after		only			statement 1	Process	disruption			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7444_s_142	9819430	(B) The dominant interfering YPT1-N22 protein binds DSS4 under conditions where the interaction of wild-type YPT1 and DSS4 is disrupted.	bind
13043	1	4240	7	11	NULL	NULL	NULL	YPT1	GP	 dominant interfering	binds			N22		DSS4	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7444_s_142	9819430	(B) The dominant interfering YPT1-N22 protein binds DSS4 under conditions where the interaction of wild-type YPT1 and DSS4 is disrupted.	bind
13045	2	4240	7	11	NULL	NULL	NULL	YPT1	GP	Wild-type	binds					DSS4	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7444_s_142	9819430	(B) The dominant interfering YPT1-N22 protein binds DSS4 under conditions where the interaction of wild-type YPT1 and DSS4 is disrupted.	bind
13047	3	4240	7	11	NULL	NULL	NULL	statement 1	Process		occurs upon					statement 2	Process	disrupted			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7444_s_142	9819430	(B) The dominant interfering YPT1-N22 protein binds DSS4 under conditions where the interaction of wild-type YPT1 and DSS4 is disrupted.	bind
12635	1	4242	5	11	NULL	NULL	NULL	MutS	GP		bind					G/T mismatch DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_233_s_112	12887908	(B) The effect of ATP and ATP S on the stability of the MutS bound to G/T mismatch DNA.	bind
13048	1	4242	7	11	NULL	NULL	NULL	MutS 	GP		bind					G/T mismatch DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_233_s_112	12887908	(B) The effect of ATP and ATP S on the stability of the MutS bound to G/T mismatch DNA.	bind
12636	1	4243	5	11	NULL	NULL	NULL	anti-TcpA 15 serum	CellComponent		bind					TCP	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_10_6050_s_255	15385509	(B) The effect of the D175A alteration on binding  of anti-TcpA 15 serum to TCP was tested.	bind
13050	1	4243	7	11	NULL	NULL	NULL	anti-TcpA 15 serum	CellComponent		bind					TCP	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_10_6050_s_255	15385509	(B) The effect of the D175A alteration on binding  of anti-TcpA 15 serum to TCP was tested.	bind
12637	1	4244	5	11	NULL	NULL	NULL	ELT-2 GATA factor protein	GP		bind		specifically			pho-1	GP	critical		GATA1 site in promoter	NULL		NULL	NULL	NULL	NULL	gw70_devbiol_279_2_446_s_181	15733671	(B) The ELT-2 GATA factor protein binds specifically  to the critical GATA1 site in the  pho-1 promoter.	bind
13053	1	4244	7	11	NULL	NULL	NULL	ELT-2 GATA factor	GP		binds		specifically			pho-1	GP			critical GATA1 site in the promoter of 	NULL		NULL	NULL	NULL	NULL	gw70_devbiol_279_2_446_s_181	15733671	(B) The ELT-2 GATA factor protein binds specifically  to the critical GATA1 site in the  pho-1 promoter.	bind
12825	1	4245	5	11	NULL	NULL	NULL	Pac-525	amino acid		bind					SDS	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_1_328_s_191	16352849	(B) The final refined average structure for Pac-525 bound to SDS.	bind
13054	1	4245	7	11	NULL	NULL	NULL	Pac-525	amino acid		bind					SDS	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_1_328_s_191	16352849	(B) The final refined average structure for Pac-525 bound to SDS.	bind
12826	1	4247	5	11	NULL	NULL	NULL	XylRdeltaA	GP		bind					restriction fragments	NucleicAcid			Pu enhancer	NULL		NULL	NULL	NULL	NULL	gw60_cell_86_2_331_s_63	8706137	(B) The footprints  shown are the result of the binding of 0.5 muM XylRdeltaA to  restriction fragments spanning exclusively the  Pu enhancer, in the presence of 5 mM  of each of the nucleotides indicated.	bind
13079	1	4247	7	11	NULL	NULL	NULL	 XylRdeltaA	GP		bind					restriction fragments	NucleicAcid	  		Pu enhancer	NULL		NULL	NULL	NULL	NULL	gw60_cell_86_2_331_s_63	8706137	(B) The footprints  shown are the result of the binding of 0.5 muM XylRdeltaA to  restriction fragments spanning exclusively the  Pu enhancer, in the presence of 5 mM  of each of the nucleotides indicated.	bind
13454	1	4249	5	11	NULL	NULL	NULL	I4AA	Chemical		is					imidazol-4-acetic acid	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_37_9_1111_s_115	9833641	(B) The GABA-C receptor antagonist imidazol-4-acetic acid (I4AA, 3 mM) caused a GABA-A mediated depression of the fEPSP slope (42%) and GABA (3 mM) applied in conjunction with I4AA led to a further 22% inhibition ( n=9).	bind
13455	2	4249	5	11	NULL	NULL	NULL	I4AA	Chemical		antagonist of					GABA-C receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_37_9_1111_s_115	9833641	(B) The GABA-C receptor antagonist imidazol-4-acetic acid (I4AA, 3 mM) caused a GABA-A mediated depression of the fEPSP slope (42%) and GABA (3 mM) applied in conjunction with I4AA led to a further 22% inhibition ( n=9).	bind
13456	3	4249	5	11	NULL	NULL	NULL	GABA	Chemical		mediate					fEPSP	Chemical	depression of			NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_37_9_1111_s_115	9833641	(B) The GABA-C receptor antagonist imidazol-4-acetic acid (I4AA, 3 mM) caused a GABA-A mediated depression of the fEPSP slope (42%) and GABA (3 mM) applied in conjunction with I4AA led to a further 22% inhibition ( n=9).	bind
13457	4	4249	5	11	NULL	NULL	NULL	I4AA	Chemical		caused					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_37_9_1111_s_115	9833641	(B) The GABA-C receptor antagonist imidazol-4-acetic acid (I4AA, 3 mM) caused a GABA-A mediated depression of the fEPSP slope (42%) and GABA (3 mM) applied in conjunction with I4AA led to a further 22% inhibition ( n=9).	bind
13458	5	4249	5	11	NULL	NULL	NULL	GABA	Chemical		inhibit		further			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_37_9_1111_s_115	9833641	(B) The GABA-C receptor antagonist imidazol-4-acetic acid (I4AA, 3 mM) caused a GABA-A mediated depression of the fEPSP slope (42%) and GABA (3 mM) applied in conjunction with I4AA led to a further 22% inhibition ( n=9).	bind
44433	6	4249	5	11	NULL	NULL	NULL	statement 5	Process		occurs in conjunction with 					I4AA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_37_9_1111_s_115	9833641	(B) The GABA-C receptor antagonist imidazol-4-acetic acid (I4AA, 3 mM) caused a GABA-A mediated depression of the fEPSP slope (42%) and GABA (3 mM) applied in conjunction with I4AA led to a further 22% inhibition ( n=9).	bind
13080	3	4249	7	11	NULL	NULL	NULL	imidazol-4-acetic acid	Chemical		cause					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_37_9_1111_s_115	9833641	(B) The GABA-C receptor antagonist imidazol-4-acetic acid (I4AA, 3 mM) caused a GABA-A mediated depression of the fEPSP slope (42%) and GABA (3 mM) applied in conjunction with I4AA led to a further 22% inhibition ( n=9).	bind
44410	1	4249	7	11	NULL	NULL	NULL	imidazol-4-acetic acid	Chemical		is an antagonist of					GABA-C receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_37_9_1111_s_115	9833641	(B) The GABA-C receptor antagonist imidazol-4-acetic acid (I4AA, 3 mM) caused a GABA-A mediated depression of the fEPSP slope (42%) and GABA (3 mM) applied in conjunction with I4AA led to a further 22% inhibition ( n=9).	bind
44411	2	4249	7	11	NULL	NULL	NULL	GABA-A 	Chemical		mediate					fEPSP	Chemical	depression of			NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_37_9_1111_s_115	9833641	(B) The GABA-C receptor antagonist imidazol-4-acetic acid (I4AA, 3 mM) caused a GABA-A mediated depression of the fEPSP slope (42%) and GABA (3 mM) applied in conjunction with I4AA led to a further 22% inhibition ( n=9).	bind
44412	4	4249	7	11	NULL	NULL	NULL	imidazol-4-acetic acid	Chemical		is					I4AA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_37_9_1111_s_115	9833641	(B) The GABA-C receptor antagonist imidazol-4-acetic acid (I4AA, 3 mM) caused a GABA-A mediated depression of the fEPSP slope (42%) and GABA (3 mM) applied in conjunction with I4AA led to a further 22% inhibition ( n=9).	bind
12827	1	4250	5	11	NULL	NULL	NULL	GST-RMP probe	GP		bind		specifically			RPB5	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7546_s_164	9819440	(B) The GST-RMP probe bound specifically to RPB5 but not to HBx, CTD, TBP, or GST.	bind
12828	2	4250	5	11	NULL	NULL	NULL	GST-RMP probe	GP		does not bind					HBx	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7546_s_164	9819440	(B) The GST-RMP probe bound specifically to RPB5 but not to HBx, CTD, TBP, or GST.	bind
12829	3	4250	5	11	NULL	NULL	NULL	GST-RMP probe	GP		does not bind								CTD		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7546_s_164	9819440	(B) The GST-RMP probe bound specifically to RPB5 but not to HBx, CTD, TBP, or GST.	bind
12830	4	4250	5	11	NULL	NULL	NULL	GST-RMP probe	GP		does not bind					TBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7546_s_164	9819440	(B) The GST-RMP probe bound specifically to RPB5 but not to HBx, CTD, TBP, or GST.	bind
12831	5	4250	5	11	NULL	NULL	NULL	GST-RMP probe	GP		does not bind					GST	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7546_s_164	9819440	(B) The GST-RMP probe bound specifically to RPB5 but not to HBx, CTD, TBP, or GST.	bind
13081	1	4250	7	11	NULL	NULL	NULL	GST-RMP probe	GP		bind		specifically			RPB5	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7546_s_164	9819440	(B) The GST-RMP probe bound specifically to RPB5 but not to HBx, CTD, TBP, or GST.	bind
13082	2	4250	7	11	NULL	NULL	NULL	GST-RMP probe	GP		does not bind					HBx	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7546_s_164	9819440	(B) The GST-RMP probe bound specifically to RPB5 but not to HBx, CTD, TBP, or GST.	bind
13083	3	4250	7	11	NULL	NULL	NULL	GST-RMP probe	GP		does not bind								CTD		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7546_s_164	9819440	(B) The GST-RMP probe bound specifically to RPB5 but not to HBx, CTD, TBP, or GST.	bind
13084	4	4250	7	11	NULL	NULL	NULL	GST-RMP probe	GP		does not bind					TBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7546_s_164	9819440	(B) The GST-RMP probe bound specifically to RPB5 but not to HBx, CTD, TBP, or GST.	bind
13085	5	4250	7	11	NULL	NULL	NULL	GST-RMP probe	GP		does not bind					GST	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7546_s_164	9819440	(B) The GST-RMP probe bound specifically to RPB5 but not to HBx, CTD, TBP, or GST.	bind
12832	1	4251	5	11	NULL	NULL	NULL	Tub2	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_175_1_17_s_29	17030980	(B) The GTP-binding pocket  of Tub2.	bind
13086	1	4251	7	11	NULL	NULL	NULL	GTP	Chemical		bind					Tub2	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_175_1_17_s_29	17030980	(B) The GTP-binding pocket  of Tub2.	bind
12833	1	4252	5	11	NULL	NULL	NULL	HOXD4	GP		bind			homeodomain		CBP	GP		HAT domain		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_21_7509_s_250	11585930	(B) The HOXD4 homeodomain binds to the CBP HAT domain.	bind
13087	1	4252	7	11	NULL	NULL	NULL	HOXD4 	GP		bind			homeodomain		CBP	GP		HAT domain		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_21_7509_s_250	11585930	(B) The HOXD4 homeodomain binds to the CBP HAT domain.	bind
12834	1	4253	5	11	NULL	NULL	NULL	Chl4p	GP		interact with					CEN DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_2_460_s_104	12589047	(B) The interaction of Chl4p with  CEN DNA depends on Ndc10p.	bind
12835	2	4253	5	11	NULL	NULL	NULL	statement 1	Process		depends on					Ndc10p	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_2_460_s_104	12589047	(B) The interaction of Chl4p with  CEN DNA depends on Ndc10p.	bind
13088	1	4253	7	11	NULL	NULL	NULL	Chl4p 	GP		bind					CEN DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_2_460_s_104	12589047	(B) The interaction of Chl4p with  CEN DNA depends on Ndc10p.	bind
13089	2	4253	7	11	NULL	NULL	NULL	statement 1	Process		depends on					Ndc10p	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_2_460_s_104	12589047	(B) The interaction of Chl4p with  CEN DNA depends on Ndc10p.	bind
12836	1	4255	5	11	NULL	NULL	NULL	alpha-actinin	GP	isolated	bind		homogenously	ABD		F-actin	GP				NULL	in resting cells 	NULL	NULL	NULL	NULL	gw60_molbiolcell_14_6_2482_s_99	12808045	(B) The isolated ABD of  alpha-actinin binds almost homogenously to F-actin in resting cells (top  row).	bind
13090	1	4255	7	11	NULL	NULL	NULL	alpha-actinin	GP	isolated	binds		homogenously	ABD		F-actin	GP	 			NULL	resting cells	NULL	NULL	NULL	NULL	gw60_molbiolcell_14_6_2482_s_99	12808045	(B) The isolated ABD of  alpha-actinin binds almost homogenously to F-actin in resting cells (top  row).	bind
12837	1	4256	5	11	NULL	NULL	NULL	PTB	GP		bind					DCS RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_20_7463_s_437	11003644	(B) The left panel shows that hnRNP H enhances PTB and nPTB binding to the DCS RNA.	bind
12838	2	4256	5	11	NULL	NULL	NULL	hnRNP H	GP		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_20_7463_s_437	11003644	(B) The left panel shows that hnRNP H enhances PTB and nPTB binding to the DCS RNA.	bind
12839	3	4256	5	11	NULL	NULL	NULL	nPTB	GP		bind					DCS RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_20_7463_s_437	11003644	(B) The left panel shows that hnRNP H enhances PTB and nPTB binding to the DCS RNA.	bind
12840	4	4256	5	11	NULL	NULL	NULL	hnRNP H	GP		enhances					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_20_7463_s_437	11003644	(B) The left panel shows that hnRNP H enhances PTB and nPTB binding to the DCS RNA.	bind
13091	1	4256	7	11	NULL	NULL	NULL	PTB 	GP		bind					DCS RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_20_7463_s_437	11003644	(B) The left panel shows that hnRNP H enhances PTB and nPTB binding to the DCS RNA.	bind
13092	2	4256	7	11	NULL	NULL	NULL	nPTB	GP		bind					DCS RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_20_7463_s_437	11003644	(B) The left panel shows that hnRNP H enhances PTB and nPTB binding to the DCS RNA.	bind
13093	3	4256	7	11	NULL	NULL	NULL	 hnRNP H	GP		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_20_7463_s_437	11003644	(B) The left panel shows that hnRNP H enhances PTB and nPTB binding to the DCS RNA.	bind
13094	4	4256	7	11	NULL	NULL	NULL	hnRNP H	GP		enhances					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_20_7463_s_437	11003644	(B) The left panel shows that hnRNP H enhances PTB and nPTB binding to the DCS RNA.	bind
12841	1	4257	5	11	NULL	NULL	NULL	cyt-PTP molecule	GP		bind		intramolecular	D1 domain		cyt-PTP molecule	GP		D2 domain		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_15_5460_s_314	12861030	(B) The less favored possibility of  intramolecular binding between D1 and D2 domains within a single cyt-PTP  molecule, which inhibits cyt-PTP  activity.	bind
12843	2	4257	5	11	NULL	NULL	NULL	statement 1	Process		inhibit					cyt-PTP	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_15_5460_s_314	12861030	(B) The less favored possibility of  intramolecular binding between D1 and D2 domains within a single cyt-PTP  molecule, which inhibits cyt-PTP  activity.	bind
13095	1	4257	7	11	NULL	NULL	NULL	 cyt-PTP molecule	GP		bind		 intramolecular	D1		 cyt-PTP molecule	GP		D2		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_15_5460_s_314	12861030	(B) The less favored possibility of  intramolecular binding between D1 and D2 domains within a single cyt-PTP  molecule, which inhibits cyt-PTP  activity.	bind
13096	2	4257	7	11	NULL	NULL	NULL	statement 1	Process		inhibits					cyt-PTP 	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_15_5460_s_314	12861030	(B) The less favored possibility of  intramolecular binding between D1 and D2 domains within a single cyt-PTP  molecule, which inhibits cyt-PTP  activity.	bind
12844	1	4261	5	11	NULL	NULL	NULL	MS2-RS domain hybrid proteins	GP		bind		specifically			MS2 RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_5_765_s_62	9660960	(B) The MS2-RS domain hybrid proteins bind specifically to MS2 RNA.	bind
13097	1	4261	7	11	NULL	NULL	NULL	MS2-RS domain hybrid protein	GP		bind		specifically			MS2 RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_5_765_s_62	9660960	(B) The MS2-RS domain hybrid proteins bind specifically to MS2 RNA.	bind
12845	1	4262	5	11	NULL	NULL	NULL	Neb1 protein	GP		bind		directly			NS1 protein	GP	viral	effector domain		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcell_1_7_991_s_44	9651582	(B) The Neb1 protein binds directly to the effector domain of the viral NS1 protein in vitro.	bind
13098	1	4262	7	11	NULL	NULL	NULL	Neb1 protein	GP		binds		directly			 NS1	GP	viral	effector domain		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcell_1_7_991_s_44	9651582	(B) The Neb1 protein binds directly to the effector domain of the viral NS1 protein in vitro.	bind
12846	1	4267	5	11	NULL	NULL	NULL	PLD1	GP		bind		specifically	PH domain		lipid monolayers	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_1_43_s_62	10660303	(b) The PH domain of PLD1 bound specifically to PI(4,5)P2-containing supported lipid monolayers.	bind
43532	2	4267	5	11	NULL	NULL	NULL	lipid monolayers	Chemical		contains					PI(4,5)P2	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_1_43_s_62	10660303	(b) The PH domain of PLD1 bound specifically to PI(4,5)P2-containing supported lipid monolayers.	bind
43533	3	4267	5	11	NULL	NULL	NULL	statement 1	Process		occurs simultaneously with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_1_43_s_62	10660303	(b) The PH domain of PLD1 bound specifically to PI(4,5)P2-containing supported lipid monolayers.	bind
13100	1	4267	7	11	NULL	NULL	NULL	PLD1	GP		bind		specifically	PH domain		PI(4,5)P2	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_1_43_s_62	10660303	(b) The PH domain of PLD1 bound specifically to PI(4,5)P2-containing supported lipid monolayers.	bind
13101	2	4267	7	11	NULL	NULL	NULL	lipid monolayers	Chemical		contain					PI(4,5)P2	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_1_43_s_62	10660303	(b) The PH domain of PLD1 bound specifically to PI(4,5)P2-containing supported lipid monolayers.	bind
43552	3	4267	7	11	NULL	NULL	NULL	statement 1	Process		occur simultaneously with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_1_43_s_62	10660303	(b) The PH domain of PLD1 bound specifically to PI(4,5)P2-containing supported lipid monolayers.	bind
12847	1	4268	5	11	NULL	NULL	NULL	ARF1	GP		bind			active site		GTP analog	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_95_2_237_s_84	9790530	(B) The picture shows the active site region of the overlapped structures of  ARF1 bound to GTP analog (yellow) or GDP (blue).	bind
12848	2	4268	5	11	NULL	NULL	NULL	ARF1	GP		bind			active site		GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_95_2_237_s_84	9790530	(B) The picture shows the active site region of the overlapped structures of  ARF1 bound to GTP analog (yellow) or GDP (blue).	bind
54273	3	4268	5	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_95_2_237_s_84	9790530	(B) The picture shows the active site region of the overlapped structures of  ARF1 bound to GTP analog (yellow) or GDP (blue).	bind
13102	1	4268	7	11	NULL	NULL	NULL	 ARF1	GP		binds			active site		GTP analog	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_95_2_237_s_84	9790530	(B) The picture shows the active site region of the overlapped structures of  ARF1 bound to GTP analog (yellow) or GDP (blue).	bind
13103	2	4268	7	11	NULL	NULL	NULL	ARF1	GP		bind			active site		GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_95_2_237_s_84	9790530	(B) The picture shows the active site region of the overlapped structures of  ARF1 bound to GTP analog (yellow) or GDP (blue).	bind
13104	3	4268	7	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_95_2_237_s_84	9790530	(B) The picture shows the active site region of the overlapped structures of  ARF1 bound to GTP analog (yellow) or GDP (blue).	bind
12849	1	4269	5	11	NULL	NULL	NULL	DRIP205	GP		bind					PPARgamma-RXR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_21_8008_s_146	11027271	(B) The PPARgamma AF-2 mutation abolishes DRIP205, but not SRC-1 or ACTR binding to PPARgamma-RXR.	bind
12850	2	4269	5	11	NULL	NULL	NULL	PPARgamma	GP	mutant	abolish			AF-2		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_21_8008_s_146	11027271	(B) The PPARgamma AF-2 mutation abolishes DRIP205, but not SRC-1 or ACTR binding to PPARgamma-RXR.	bind
12851	3	4269	5	11	NULL	NULL	NULL	SRC-1	GP		bind					PPARgamma-RXR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_21_8008_s_146	11027271	(B) The PPARgamma AF-2 mutation abolishes DRIP205, but not SRC-1 or ACTR binding to PPARgamma-RXR.	bind
12852	4	4269	5	11	NULL	NULL	NULL	PPARgamma	GP	mutant	does not abolish			AF-2		statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_21_8008_s_146	11027271	(B) The PPARgamma AF-2 mutation abolishes DRIP205, but not SRC-1 or ACTR binding to PPARgamma-RXR.	bind
12853	5	4269	5	11	NULL	NULL	NULL	ACTR	GP		bind					PPARgamma-RXR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_21_8008_s_146	11027271	(B) The PPARgamma AF-2 mutation abolishes DRIP205, but not SRC-1 or ACTR binding to PPARgamma-RXR.	bind
12854	6	4269	5	11	NULL	NULL	NULL	PPARgamma	GP	mutant	does not abolish			AF-2		statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_21_8008_s_146	11027271	(B) The PPARgamma AF-2 mutation abolishes DRIP205, but not SRC-1 or ACTR binding to PPARgamma-RXR.	bind
13106	1	4269	7	11	NULL	NULL	NULL	DRIP205	GP		bind					PPARgamma-RXR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_21_8008_s_146	11027271	(B) The PPARgamma AF-2 mutation abolishes DRIP205, but not SRC-1 or ACTR binding to PPARgamma-RXR.	bind
13107	2	4269	7	11	NULL	NULL	NULL	SRC-1	GP		bind					PPARgamma-RXR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_21_8008_s_146	11027271	(B) The PPARgamma AF-2 mutation abolishes DRIP205, but not SRC-1 or ACTR binding to PPARgamma-RXR.	bind
13108	3	4269	7	11	NULL	NULL	NULL	ACTR	GP		bind					PPARgamma-RXR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_21_8008_s_146	11027271	(B) The PPARgamma AF-2 mutation abolishes DRIP205, but not SRC-1 or ACTR binding to PPARgamma-RXR.	bind
13109	4	4269	7	11	NULL	NULL	NULL	PPARgamma	GP	mutation of	abolishes			AF-2		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_21_8008_s_146	11027271	(B) The PPARgamma AF-2 mutation abolishes DRIP205, but not SRC-1 or ACTR binding to PPARgamma-RXR.	bind
13110	5	4269	7	11	NULL	NULL	NULL	PPARgamma	GP	mutation of	does not abolish			AF-2		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_21_8008_s_146	11027271	(B) The PPARgamma AF-2 mutation abolishes DRIP205, but not SRC-1 or ACTR binding to PPARgamma-RXR.	bind
13111	6	4269	7	11	NULL	NULL	NULL	PPARgamma	GP	mutation of	does not abolish			AF-2		statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_21_8008_s_146	11027271	(B) The PPARgamma AF-2 mutation abolishes DRIP205, but not SRC-1 or ACTR binding to PPARgamma-RXR.	bind
12855	1	4270	5	11	NULL	NULL	NULL	Grb2	GP		bind					Gab2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3744_s_53	11997510	(B) The PRD is sufficient to mediate binding of Grb2 and Mona to either Gab2 or Gab3.	bind
12856	2	4270	5	11	NULL	NULL	NULL	Grb2	GP		bind					Gab3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3744_s_53	11997510	(B) The PRD is sufficient to mediate binding of Grb2 and Mona to either Gab2 or Gab3.	bind
12857	3	4270	5	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3744_s_53	11997510	(B) The PRD is sufficient to mediate binding of Grb2 and Mona to either Gab2 or Gab3.	bind
12858	4	4270	5	11	NULL	NULL	NULL				mediates			PRD		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3744_s_53	11997510	(B) The PRD is sufficient to mediate binding of Grb2 and Mona to either Gab2 or Gab3.	bind
12859	5	4270	5	11	NULL	NULL	NULL				mediates			PRD		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3744_s_53	11997510	(B) The PRD is sufficient to mediate binding of Grb2 and Mona to either Gab2 or Gab3.	bind
12860	6	4270	5	11	NULL	NULL	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3744_s_53	11997510	(B) The PRD is sufficient to mediate binding of Grb2 and Mona to either Gab2 or Gab3.	bind
12861	7	4270	5	11	NULL	NULL	NULL	Mona	GP		bind					Gab2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3744_s_53	11997510	(B) The PRD is sufficient to mediate binding of Grb2 and Mona to either Gab2 or Gab3.	bind
12862	8	4270	5	11	NULL	NULL	NULL	Mona	GP		bind					Gab3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3744_s_53	11997510	(B) The PRD is sufficient to mediate binding of Grb2 and Mona to either Gab2 or Gab3.	bind
12863	9	4270	5	11	NULL	NULL	NULL	statement 7	Process		is an alternative to					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3744_s_53	11997510	(B) The PRD is sufficient to mediate binding of Grb2 and Mona to either Gab2 or Gab3.	bind
12864	10	4270	5	11	NULL	NULL	NULL				mediates			PRD		statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3744_s_53	11997510	(B) The PRD is sufficient to mediate binding of Grb2 and Mona to either Gab2 or Gab3.	bind
12865	11	4270	5	11	NULL	NULL	NULL				mediates			PRD		statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3744_s_53	11997510	(B) The PRD is sufficient to mediate binding of Grb2 and Mona to either Gab2 or Gab3.	bind
12866	12	4270	5	11	NULL	NULL	NULL	statement 10	Process		is an alternative to					statement 11	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3744_s_53	11997510	(B) The PRD is sufficient to mediate binding of Grb2 and Mona to either Gab2 or Gab3.	bind
13112	1	4270	7	11	NULL	NULL	NULL	Grb2 	GP		bind					Gab2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3744_s_53	11997510	(B) The PRD is sufficient to mediate binding of Grb2 and Mona to either Gab2 or Gab3.	bind
13113	2	4270	7	11	NULL	NULL	NULL	Mona	GP		bind					Gab2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3744_s_53	11997510	(B) The PRD is sufficient to mediate binding of Grb2 and Mona to either Gab2 or Gab3.	bind
13114	3	4270	7	11	NULL	NULL	NULL	Grb2 	GP		bind					Gab3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3744_s_53	11997510	(B) The PRD is sufficient to mediate binding of Grb2 and Mona to either Gab2 or Gab3.	bind
13115	4	4270	7	11	NULL	NULL	NULL	Mona	GP		bind					Gab3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3744_s_53	11997510	(B) The PRD is sufficient to mediate binding of Grb2 and Mona to either Gab2 or Gab3.	bind
13116	5	4270	7	11	NULL	NULL	NULL				mediates			PRD		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3744_s_53	11997510	(B) The PRD is sufficient to mediate binding of Grb2 and Mona to either Gab2 or Gab3.	bind
13117	6	4270	7	11	NULL	NULL	NULL				mediates			PRD		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3744_s_53	11997510	(B) The PRD is sufficient to mediate binding of Grb2 and Mona to either Gab2 or Gab3.	bind
13118	7	4270	7	11	NULL	NULL	NULL				mediates			PRD		statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3744_s_53	11997510	(B) The PRD is sufficient to mediate binding of Grb2 and Mona to either Gab2 or Gab3.	bind
13119	8	4270	7	11	NULL	NULL	NULL				mediates			PRD		statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3744_s_53	11997510	(B) The PRD is sufficient to mediate binding of Grb2 and Mona to either Gab2 or Gab3.	bind
54274	9	4270	7	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3744_s_53	11997510	(B) The PRD is sufficient to mediate binding of Grb2 and Mona to either Gab2 or Gab3.	bind
54275	10	4270	7	11	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3744_s_53	11997510	(B) The PRD is sufficient to mediate binding of Grb2 and Mona to either Gab2 or Gab3.	bind
54276	11	4270	7	11	NULL	NULL	NULL	statement 5	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3744_s_53	11997510	(B) The PRD is sufficient to mediate binding of Grb2 and Mona to either Gab2 or Gab3.	bind
54277	12	4270	7	11	NULL	NULL	NULL	statement 7	Process		is an alternative to					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3744_s_53	11997510	(B) The PRD is sufficient to mediate binding of Grb2 and Mona to either Gab2 or Gab3.	bind
12867	1	4271	5	11	NULL	NULL	NULL	Reelin	GP		bind					VLDLR-expressing cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_neuron_24_2_471_s_127	10571240	(B) The relative amount of Reelin bound to VLDLR-expressing cells from two independent experiments was plotted against the concentration of Reelin (nM).	bind
13120	2	4271	7	11	NULL	NULL	NULL	Reelin 	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_24_2_471_s_127	10571240	(B) The relative amount of Reelin bound to VLDLR-expressing cells from two independent experiments was plotted against the concentration of Reelin (nM).	bind
44413	1	4271	7	11	NULL	NULL	NULL	cells	cell		express					VLDLR	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_24_2_471_s_127	10571240	(B) The relative amount of Reelin bound to VLDLR-expressing cells from two independent experiments was plotted against the concentration of Reelin (nM).	bind
12868	1	4275	5	11	NULL	NULL	NULL				bind			SWI/SNF subunit		SNZ1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8829_s_134	14612422	(B) The same process was used as for panel A except that  the SWI/SNF subunit binding to the  SNZ1 promoter was analyzed.	bind
13121	1	4275	7	11	NULL	NULL	NULL				bind			SWI/SNF subunit		 SNZ1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8829_s_134	14612422	(B) The same process was used as for panel A except that  the SWI/SNF subunit binding to the  SNZ1 promoter was analyzed.	bind
16449	1	4278	5	11	NULL	NULL	NULL	Pol II	GP		bind					GAL10	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_5_1301_s_135	12769853	(B) The strain was deleted for  gal11, and the binding of Pol II and of SAGA was measured at the  GAL10 promoter following induction.	bind
16451	2	4278	5	11	NULL	NULL	NULL	SAGA	GP		bind					GAL10	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_5_1301_s_135	12769853	(B) The strain was deleted for  gal11, and the binding of Pol II and of SAGA was measured at the  GAL10 promoter following induction.	bind
13336	1	4278	7	11	NULL	NULL	NULL	 Pol II	GP		bind					GAL10	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_5_1301_s_135	12769853	(B) The strain was deleted for  gal11, and the binding of Pol II and of SAGA was measured at the  GAL10 promoter following induction.	bind
13337	2	4278	7	11	NULL	NULL	NULL	SAGA	GP		bind					GAL10	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_5_1301_s_135	12769853	(B) The strain was deleted for  gal11, and the binding of Pol II and of SAGA was measured at the  GAL10 promoter following induction.	bind
16453	1	4281	5	11	NULL	NULL	NULL	Ubc9	GP		bind					Nup358	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6498_s_264	12192048	(B) The synergistic effect of SUMO-1-modified RanGAP1 on the binding of Ubc9 to Nup358 was investigated.	bind
16454	2	4281	5	11	NULL	NULL	NULL	RanGAP1 	GP	SUMO-1-modified	effect		synergistically			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6498_s_264	12192048	(B) The synergistic effect of SUMO-1-modified RanGAP1 on the binding of Ubc9 to Nup358 was investigated.	bind
13124	1	4281	7	11	NULL	NULL	NULL	Ubc9	GP		bind					Nup358	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6498_s_264	12192048	(B) The synergistic effect of SUMO-1-modified RanGAP1 on the binding of Ubc9 to Nup358 was investigated.	bind
13125	2	4281	7	11	NULL	NULL	NULL	RanGAP1 	GP	SUMO-1-modified	effect		synergistically			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6498_s_264	12192048	(B) The synergistic effect of SUMO-1-modified RanGAP1 on the binding of Ubc9 to Nup358 was investigated.	bind
16455	1	4282	5	11	NULL	NULL	NULL	F1 phage	Organism		bind					AMA1	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_10_6981_s_147	16177378	(B) The synthetic peptides R1, F1, and F1(s), a scrambled  version of the F1 peptide, were tested for their ability to block binding of F1 phage  to AMA1.	bind
13126	1	4282	7	11	NULL	NULL	NULL	F1 phage	Organism		bind					AMA1	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_10_6981_s_147	16177378	(B) The synthetic peptides R1, F1, and F1(s), a scrambled  version of the F1 peptide, were tested for their ability to block binding of F1 phage  to AMA1.	bind
16456	2	4283	5	11	NULL	NULL	NULL	TNFR2	GP		is required for			TRAF2 binding region		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_11_6_783_s_83	10626900	(B) The TRAF2 binding region of TNFR2 is required for TNF-mediated cell death.	bind
44434	1	4283	5	11	NULL	NULL	NULL	TNF	GP		mediate					cell death	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_11_6_783_s_83	10626900	(B) The TRAF2 binding region of TNFR2 is required for TNF-mediated cell death.	bind
13127	2	4283	7	11	NULL	NULL	NULL	TNFR2	GP		is required for			TRAF2 binding region		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_11_6_783_s_83	10626900	(B) The TRAF2 binding region of TNFR2 is required for TNF-mediated cell death.	bind
44414	1	4283	7	11	NULL	NULL	NULL	TNF	GP		mediate					cell death	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_11_6_783_s_83	10626900	(B) The TRAF2 binding region of TNFR2 is required for TNF-mediated cell death.	bind
16457	1	4284	5	11	NULL	NULL	NULL	TCR	GP		bind			V domain		HLA-A2	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_8_4_403_s_43	9586631	(B) The V  and V  domains of each TCR bound to HLA-A2 (colors as in	bind
13128	1	4284	7	11	NULL	NULL	NULL	 TCR 	GP		binds			V and V domain		HLA-A2	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_8_4_403_s_43	9586631	(B) The V  and V  domains of each TCR bound to HLA-A2 (colors as in	bind
16458	1	4286	5	11	NULL	NULL	NULL	Stat3	GP	mutant	bind		decreased			c-Jun	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_7138_s_135	10490649	(B) Three Stat3 mutants showed decreased c-Jun binding.	bind
13129	1	4286	7	11	NULL	NULL	NULL	Stat3	GP	mutant	bind		decreased			c-Jun	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_7138_s_135	10490649	(B) Three Stat3 mutants showed decreased c-Jun binding.	bind
16459	1	4288	5	11	NULL	NULL	NULL	125I-P40	GP		bind					CEM cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_9_4456_s_120	10456886	(B) Time course of 125I-P40 (106 cpm; 10 9 M) binding to CEM cells (8 x 106).	bind
13130	1	4288	7	11	NULL	NULL	NULL	125I-P40 	GP		bind					CEM cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_9_4456_s_120	10456886	(B) Time course of 125I-P40 (106 cpm; 10 9 M) binding to CEM cells (8 x 106).	bind
16460	2	4289	5	11	NULL	NULL	NULL	[3]AII	GP		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_8_1495_s_179	12721105	(b) Time course of PMA effect on [3]AII (4 nM) binding to HEK 293 cells stably expressing AT1R - YFP. (c) Effect of PMA on [3]Lys-des-Arg9-bradykinin binding to HEK 293 cells stably expressing B1R - YFP.	bind
16461	3	4289	5	11	NULL	NULL	NULL	[3]Lys-des-Arg9-bradykinin	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_8_1495_s_179	12721105	(b) Time course of PMA effect on [3]AII (4 nM) binding to HEK 293 cells stably expressing AT1R - YFP. (c) Effect of PMA on [3]Lys-des-Arg9-bradykinin binding to HEK 293 cells stably expressing B1R - YFP.	bind
44435	1	4289	5	11	NULL	NULL	NULL	HEK 293 cells	cell		express		stably			AT1R - YFP	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_8_1495_s_179	12721105	(b) Time course of PMA effect on [3]AII (4 nM) binding to HEK 293 cells stably expressing AT1R - YFP. (c) Effect of PMA on [3]Lys-des-Arg9-bradykinin binding to HEK 293 cells stably expressing B1R - YFP.	bind
13132	2	4289	7	11	NULL	NULL	NULL	[3]AII	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_8_1495_s_179	12721105	(b) Time course of PMA effect on [3]AII (4 nM) binding to HEK 293 cells stably expressing AT1R - YFP. (c) Effect of PMA on [3]Lys-des-Arg9-bradykinin binding to HEK 293 cells stably expressing B1R - YFP.	bind
13133	3	4289	7	11	NULL	NULL	NULL	[3]Lys-des-Arg9-bradykinin	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_8_1495_s_179	12721105	(b) Time course of PMA effect on [3]AII (4 nM) binding to HEK 293 cells stably expressing AT1R - YFP. (c) Effect of PMA on [3]Lys-des-Arg9-bradykinin binding to HEK 293 cells stably expressing B1R - YFP.	bind
44415	1	4289	7	11	NULL	NULL	NULL	HEK 293 cells	cell		express		stably			AT1R - YFP	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_8_1495_s_179	12721105	(b) Time course of PMA effect on [3]AII (4 nM) binding to HEK 293 cells stably expressing AT1R - YFP. (c) Effect of PMA on [3]Lys-des-Arg9-bradykinin binding to HEK 293 cells stably expressing B1R - YFP.	bind
16462	1	4290	5	11	NULL	NULL	NULL	cPot1	GP		bind					MBS oligonucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_5_2091_s_282	14966288	(B) Titration curve for cPot1 binding to the MBS  oligonucleotide.	bind
13134	1	4290	7	11	NULL	NULL	NULL	cPot1	GP		bind					MBS oligonucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_5_2091_s_282	14966288	(B) Titration curve for cPot1 binding to the MBS  oligonucleotide.	bind
16463	1	4291	5	11	NULL	NULL	NULL	p53	GP		bind			Arg		p53CON DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_2_1092_s_174	9891044	(B) Titration of p53Pro and p53Arg binding to p53CON DNA.	bind
16464	2	4291	5	11	NULL	NULL	NULL	p53	GP		bind			Pro		p53CON DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_2_1092_s_174	9891044	(B) Titration of p53Pro and p53Arg binding to p53CON DNA.	bind
13135	1	4291	7	11	NULL	NULL	NULL	p53	GP		bind			Pro		p53CON DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_2_1092_s_174	9891044	(B) Titration of p53Pro and p53Arg binding to p53CON DNA.	bind
13136	2	4291	7	11	NULL	NULL	NULL	p53	GP		bind			Arg		p53CON DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_2_1092_s_174	9891044	(B) Titration of p53Pro and p53Arg binding to p53CON DNA.	bind
16465	1	4292	5	11	NULL	NULL	NULL	TM-1	GP		does not bind					B7-1	Cell				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_5_11_1303_s_166	8574588	(b) TM-1 does not bind to B7-1, B7-2 or ICAM-1, as determined by flow cytometry.	bind
16466	2	4292	5	11	NULL	NULL	NULL	TM-1	GP		does not bind					B7-2	Cell				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_5_11_1303_s_166	8574588	(b) TM-1 does not bind to B7-1, B7-2 or ICAM-1, as determined by flow cytometry.	bind
16467	3	4292	5	11	NULL	NULL	NULL	TM-1	GP		does not bind					ICAM-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_5_11_1303_s_166	8574588	(b) TM-1 does not bind to B7-1, B7-2 or ICAM-1, as determined by flow cytometry.	bind
13137	1	4292	7	11	NULL	NULL	NULL	TM-1	GP		does not bind					B7-1	Cell				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_5_11_1303_s_166	8574588	(b) TM-1 does not bind to B7-1, B7-2 or ICAM-1, as determined by flow cytometry.	bind
13138	2	4292	7	11	NULL	NULL	NULL	TM-1	GP		does not bind					B7-2	Cell				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_5_11_1303_s_166	8574588	(b) TM-1 does not bind to B7-1, B7-2 or ICAM-1, as determined by flow cytometry.	bind
13139	3	4292	7	11	NULL	NULL	NULL	TM-1	GP		does not bind					ICAM-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_5_11_1303_s_166	8574588	(b) TM-1 does not bind to B7-1, B7-2 or ICAM-1, as determined by flow cytometry.	bind
16468	1	4293	5	11	NULL	NULL	NULL	PIP3	GP		bind					PKB	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7794_s_199	14560023	(B) To assess the importance  of PKCzeta activation in influencing the binding of PIP3 to PKB, the experiment in panel A was repeated but with TBST buffer that either lacked  ATP, PS, and MgCl2 or which had been supplemented with Ro 31.8220 (Ro, 5 muM), as indicated.	bind
13140	1	4293	7	11	NULL	NULL	NULL	PIP3	GP		bind					PKB	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7794_s_199	14560023	(B) To assess the importance  of PKCzeta activation in influencing the binding of PIP3 to PKB, the experiment in panel A was repeated but with TBST buffer that either lacked  ATP, PS, and MgCl2 or which had been supplemented with Ro 31.8220 (Ro, 5 muM), as indicated.	bind
16469	1	4298	5	11	NULL	NULL	NULL	c-Myb proteins	GP	35S-labeled	bind					GST-KIX	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5601_s_102	10409749	(B) Top, representative autoradiogram obtained following SDS-PAGE of 35S-labeled c-Myb proteins bound to GST-KIX resin.	bind
13142	1	4298	7	11	NULL	NULL	NULL	c-Myb protein	GP	35S-labeled	bind					GST-KIX	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5601_s_102	10409749	(B) Top, representative autoradiogram obtained following SDS-PAGE of 35S-labeled c-Myb proteins bound to GST-KIX resin.	bind
16470	1	4299	5	11	NULL	NULL	NULL	c-jun	GP		bind					ET-1	GP			Ap1 element in promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_14_5518_s_174	16809784	(B) Transcription factor c-jun binds the Ap1 element in the ET-1  promoter.	bind
44436	2	4299	5	11	NULL	NULL	NULL	c-jun	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_14_5518_s_174	16809784	(B) Transcription factor c-jun binds the Ap1 element in the ET-1  promoter.	bind
13143	1	4299	7	11	NULL	NULL	NULL	c-jun	GP		binds					ET-1	GP			Ap1 element in the promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_14_5518_s_174	16809784	(B) Transcription factor c-jun binds the Ap1 element in the ET-1  promoter.	bind
44416	2	4299	7	11	NULL	NULL	NULL	c-jun	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_14_5518_s_174	16809784	(B) Transcription factor c-jun binds the Ap1 element in the ET-1  promoter.	bind
10518	1	4300	5	11	NULL	NULL	NULL	p27	GP		bind		transiently			CRM1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_1_201_s_141	12529437	(B) Transient binding of p27 to CRM1 occurs early in G1.	bind
10519	2	4300	5	11	NULL	NULL	NULL	statement 1	Process		occurs early in					G1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_1_201_s_141	12529437	(B) Transient binding of p27 to CRM1 occurs early in G1.	bind
9857	1	4300	6	11	NULL	NULL	NULL	p27	GP		bind		transiently			CRM1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_1_201_s_141	12529437	(B) Transient binding of p27 to CRM1 occurs early in G1.	bind
9858	2	4300	6	11	NULL	NULL	NULL	statement 1	Process		occurs early in					G1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_1_201_s_141	12529437	(B) Transient binding of p27 to CRM1 occurs early in G1.	bind
10520	1	4301	5	NULL	NULL	0	NULL	TRF2	NULL		bind	NULL				POT1	NULL				NULL	293 cells	0	NULL	NULL	NULL	gw70_molcellbiol_25_3_1070_s_215	15657433	(B) TRF2 and TRF2deltaBdeltaM bound to POT1 in 293 cells.	bind
10521	2	4301	5	NULL	NULL	0	NULL	TRF2deltaBdeltaM	NULL		bind	NULL				POT1	NULL				NULL	293 cells	0	NULL	NULL	NULL	gw70_molcellbiol_25_3_1070_s_215	15657433	(B) TRF2 and TRF2deltaBdeltaM bound to POT1 in 293 cells.	bind
9859	1	4301	6	NULL	NULL	0	NULL	TRF2	GP		bind					POT1	GP				NULL	293 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_3_1070_s_215	15657433	(B) TRF2 and TRF2deltaBdeltaM bound to POT1 in 293 cells.	bind
9860	2	4301	6	NULL	NULL	0	NULL	TRF2deltaBdeltaM	GP		bind					POT1	GP				NULL	293 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_3_1070_s_215	15657433	(B) TRF2 and TRF2deltaBdeltaM bound to POT1 in 293 cells.	bind
10522	1	4302	5	NULL	NULL	0	NULL	Tubulin	NULL		bind	NULL				Op18  derivatives	NULL	Flag-epitope - tagged			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_146_6_1289_s_111	10491392	(B) Tubulin binding to the indicated Op18 Flag-epitope - tagged derivatives was analyzed at equimolar concentration (10 muM) in PEM, pH 6.8, containing 17% glycerol.	bind
9861	1	4302	6	NULL	NULL	0	NULL	Tubulin	GP		bind					Op18 derivates	GP	Flag-eptitope			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_146_6_1289_s_111	10491392	(B) Tubulin binding to the indicated Op18 Flag-epitope - tagged derivatives was analyzed at equimolar concentration (10 muM) in PEM, pH 6.8, containing 17% glycerol.	bind
10526	1	4306	5	NULL	NULL	0	NULL		NULL		bind	NULL		Uba domain		polyubiquitin chains	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_9_3868_s_64	12972570	(B) Uba domain binding to polyubiquitin chains does not  correlate with proteasome pull down.	bind
11443	2	4306	5	NULL	NULL	0	NULL	statement 1	NULL		does not correlate with	NULL				proteasome	NULL	pull down of			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_9_3868_s_64	12972570	(B) Uba domain binding to polyubiquitin chains does not  correlate with proteasome pull down.	bind
9862	1	4306	6	NULL	NULL	0	NULL		NULL		bind	NULL		Uba		polyubiquitin chains	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_9_3868_s_64	12972570	(B) Uba domain binding to polyubiquitin chains does not  correlate with proteasome pull down.	bind
54260	2	4306	6	10	NULL	0	NULL	statement 1			does not correlate with					proteasome		pull down of			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_9_3868_s_64	12972570	(B) Uba domain binding to polyubiquitin chains does not  correlate with proteasome pull down.	bind
10527	1	4307	5	NULL	NULL	0	NULL	CP2	NULL		bind	NULL				GATA-1 oligonucleotide	NULL			HS2 enhancer 	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_10_3942_s_119	16648487	(B) Unlabeled  oligonucleotides comprising the wild-type (wt) or mutated GATA-1 palindrome do not  affect the binding of CP2 to the GATA-1 HS2 enhancer oligonucleotide in competition  experiments.	bind
9863	1	4307	6	NULL	NULL	0	NULL	CP2	GP		bind					GATA-1 oligonucleotide	NucleicAcid			HS2 enhancer	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_10_3942_s_119	16648487	(B) Unlabeled  oligonucleotides comprising the wild-type (wt) or mutated GATA-1 palindrome do not  affect the binding of CP2 to the GATA-1 HS2 enhancer oligonucleotide in competition  experiments.	bind
10528	1	4309	5	NULL	NULL	0	NULL	v-E10	NULL		bind	NULL		PQE binding motif		TRAF6	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_1115_s_92	11238466	(B) v-E10 binds TRAF6 via a PQE binding motif.	bind
9864	1	4309	6	NULL	NULL	0	NULL	v-E10	GP		bind			PQE binding motif		TRAF6	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_1115_s_92	11238466	(B) v-E10 binds TRAF6 via a PQE binding motif.	bind
10532	1	4310	5	NULL	NULL	0	NULL	VDE	NULL		bind	NULL				Srp1p	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_molcellbiol_23_5_1726_s_222	12588991	(B) VDE binds Srp1p in vitro.	bind
9865	1	4310	6	NULL	NULL	0	NULL	VDE	GP		bind					Srp1p	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_23_5_1726_s_222	12588991	(B) VDE binds Srp1p in vitro.	bind
10533	1	4311	5	NULL	NULL	0	NULL	VDR	NULL		is present in	NULL				Jun-Fos DNA-bound complex	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_6_4191_s_190	10330159	(B) VDR is present in the Jun-Fos DNA-bound complex.	bind
10534	1	4312	5	NULL	NULL	0	NULL	Vg	NULL		associate with	NULL				Sd	NULL				NULL		0	NULL	NULL	NULL	gw60_development_130_17_4135_s_493	12874133	(B) Vg associates with Sd to form a bipartite transcription factor (Vg/Sd) that controls the expression of an unknown diffusible factor.	bind
10627	2	4312	5	NULL	NULL	0	NULL	statement 1	NULL		forms	NULL				Vg/Sd bipartite transcription factor	NULL				NULL		NULL	NULL	NULL	NULL	gw60_development_130_17_4135_s_493	12874133	(B) Vg associates with Sd to form a bipartite transcription factor (Vg/Sd) that controls the expression of an unknown diffusible factor.	bind
10628	3	4312	5	10	NULL	0	NULL	statement 2			control					unknown diffusible factor		expression of 			NULL		NULL	NULL	NULL	NULL	gw60_development_130_17_4135_s_493	12874133	(B) Vg associates with Sd to form a bipartite transcription factor (Vg/Sd) that controls the expression of an unknown diffusible factor.	bind
9867	1	4312	6	NULL	NULL	NULL	NULL	Vg	GP		associate with					Sd	GP				NULL		NULL	NULL	NULL	NULL	gw60_development_130_17_4135_s_493	12874133	(B) Vg associates with Sd to form a bipartite transcription factor (Vg/Sd) that controls the expression of an unknown diffusible factor.	bind
9868	2	4312	6	NULL	NULL	NULL	NULL	statement 1	Process		forms					bipartite transcription factor (Vg/Sd)	GP				NULL		NULL	NULL	NULL	NULL	gw60_development_130_17_4135_s_493	12874133	(B) Vg associates with Sd to form a bipartite transcription factor (Vg/Sd) that controls the expression of an unknown diffusible factor.	bind
10630	1	4313	5	NULL	NULL	0	NULL	Vpr	NULL		bind	NULL				ANT	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_583_s_238	12729593	(B) Vpr binds to the adenine nucleotide translocator (ANT) to induce mitochondrial  membrane potential (MMP).	bind
10631	2	4313	5	NULL	NULL	0	NULL	ANT	NULL		is	NULL				adenine nucleotide translocator	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_583_s_238	12729593	(B) Vpr binds to the adenine nucleotide translocator (ANT) to induce mitochondrial  membrane potential (MMP).	bind
10632	3	4313	5	NULL	NULL	0	NULL	statement 1	NULL		induce	NULL				MMP	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_583_s_238	12729593	(B) Vpr binds to the adenine nucleotide translocator (ANT) to induce mitochondrial  membrane potential (MMP).	bind
10633	4	4313	5	NULL	NULL	0	NULL	MMP	NULL		is	NULL				mitochondrial membrane potential	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_583_s_238	12729593	(B) Vpr binds to the adenine nucleotide translocator (ANT) to induce mitochondrial  membrane potential (MMP).	bind
9870	1	4313	6	NULL	NULL	NULL	NULL	Vpr	GP		bind					ANT	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_583_s_238	12729593	(B) Vpr binds to the adenine nucleotide translocator (ANT) to induce mitochondrial  membrane potential (MMP).	bind
9871	2	4313	6	NULL	NULL	NULL	NULL	ANT	GP		is					adenine nucleotide translocator	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_583_s_238	12729593	(B) Vpr binds to the adenine nucleotide translocator (ANT) to induce mitochondrial  membrane potential (MMP).	bind
9872	3	4313	6	NULL	NULL	NULL	NULL	statement 1	Process		induce					MMP	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_583_s_238	12729593	(B) Vpr binds to the adenine nucleotide translocator (ANT) to induce mitochondrial  membrane potential (MMP).	bind
9873	4	4313	6	NULL	NULL	NULL	NULL	MMP	Process		is					mitochondrial membrane potential	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_583_s_238	12729593	(B) Vpr binds to the adenine nucleotide translocator (ANT) to induce mitochondrial  membrane potential (MMP).	bind
10635	1	4315	5	NULL	NULL	0	NULL	Vps45p	NULL		bind	NULL				Vac1p	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_9_3_159_s_68	10021387	(b) Vps45p binds Vac1p.	bind
9874	1	4315	6	NULL	NULL	NULL	NULL	Vps45p	GP		bind					Vac1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_3_159_s_68	10021387	(b) Vps45p binds Vac1p.	bind
10638	1	4316	5	NULL	NULL	0	NULL	cyclin E	NULL		bind	NULL				p107 derivatives	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_9_5380_s_295	9710622	(B) Western blot analysis of cyclin E bound to p107 derivatives.	bind
9875	1	4316	6	NULL	NULL	NULL	NULL	Cyclin E	GP		bind					p107 derivatives	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5380_s_295	9710622	(B) Western blot analysis of cyclin E bound to p107 derivatives.	bind
10642	1	4318	5	NULL	NULL	0	NULL	uPAR	NULL	occupied	bind	NULL				LRP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1467_s_304	11359936	(B) When binding of occupied uPAR to LRP is prevented, uPA:PAI-1 bridges uPAR and LRP and occupied uPAR moves into clathrin-coated pits.	bind
10643	2	4318	5	NULL	NULL	0	NULL	uPA:PAI-1	NULL		bridges	NULL				uPAR	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1467_s_304	11359936	(B) When binding of occupied uPAR to LRP is prevented, uPA:PAI-1 bridges uPAR and LRP and occupied uPAR moves into clathrin-coated pits.	bind
10644	4	4318	5	NULL	NULL	0	NULL	statement 2	NULL		in the absence of	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1467_s_304	11359936	(B) When binding of occupied uPAR to LRP is prevented, uPA:PAI-1 bridges uPAR and LRP and occupied uPAR moves into clathrin-coated pits.	bind
10647	6	4318	5	NULL	NULL	0	NULL	uPAR	NULL	occupied	moves into	NULL				clathrin-coated pits	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1467_s_304	11359936	(B) When binding of occupied uPAR to LRP is prevented, uPA:PAI-1 bridges uPAR and LRP and occupied uPAR moves into clathrin-coated pits.	bind
10650	5	4318	5	10	NULL	0	NULL	statement 3			in the absence of					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1467_s_304	11359936	(B) When binding of occupied uPAR to LRP is prevented, uPA:PAI-1 bridges uPAR and LRP and occupied uPAR moves into clathrin-coated pits.	bind
13040	3	4318	5	NULL	NULL	0	NULL	uPA:PAI-1	NULL		bridges	NULL				LRP	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_5_1467_s_304	11359936	(B) When binding of occupied uPAR to LRP is prevented, uPA:PAI-1 bridges uPAR and LRP and occupied uPAR moves into clathrin-coated pits.	bind
54261	7	4318	5	10	NULL	0	NULL	statement 6			in absence of					statement 1					NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_5_1467_s_304	11359936	(B) When binding of occupied uPAR to LRP is prevented, uPA:PAI-1 bridges uPAR and LRP and occupied uPAR moves into clathrin-coated pits.	bind
10803	1	4318	6	NULL	NULL	NULL	NULL	uPAR	GP	occupied	bind					LRP	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1467_s_304	11359936	(B) When binding of occupied uPAR to LRP is prevented, uPA:PAI-1 bridges uPAR and LRP and occupied uPAR moves into clathrin-coated pits.	bind
10804	2	4318	6	NULL	NULL	NULL	NULL	uPA:PAI-1	GP		bridges					uPAR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1467_s_304	11359936	(B) When binding of occupied uPAR to LRP is prevented, uPA:PAI-1 bridges uPAR and LRP and occupied uPAR moves into clathrin-coated pits.	bind
10805	3	4318	6	NULL	NULL	NULL	NULL	uPA:PAI-1	GP		bridges					LRP	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1467_s_304	11359936	(B) When binding of occupied uPAR to LRP is prevented, uPA:PAI-1 bridges uPAR and LRP and occupied uPAR moves into clathrin-coated pits.	bind
10806	4	4318	6	NULL	NULL	NULL	NULL	statement 2	Process		occurs in absence of					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1467_s_304	11359936	(B) When binding of occupied uPAR to LRP is prevented, uPA:PAI-1 bridges uPAR and LRP and occupied uPAR moves into clathrin-coated pits.	bind
10807	5	4318	6	NULL	NULL	NULL	NULL	statement 3	Process		occurs in absence of					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1467_s_304	11359936	(B) When binding of occupied uPAR to LRP is prevented, uPA:PAI-1 bridges uPAR and LRP and occupied uPAR moves into clathrin-coated pits.	bind
10808	6	4318	6	NULL	NULL	NULL	NULL	uPAR	GP	occupied	moves to					clathrin-coated pits	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1467_s_304	11359936	(B) When binding of occupied uPAR to LRP is prevented, uPA:PAI-1 bridges uPAR and LRP and occupied uPAR moves into clathrin-coated pits.	bind
10809	7	4318	6	NULL	NULL	NULL	NULL	statement 6	Process		occurs in absence of					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1467_s_304	11359936	(B) When binding of occupied uPAR to LRP is prevented, uPA:PAI-1 bridges uPAR and LRP and occupied uPAR moves into clathrin-coated pits.	bind
10653	1	4319	5	NULL	NULL	0	NULL	SatA	NULL		bind	NULL	tightly			SatB/atC	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_73_10_6727_s_194	16177350	(B) When SatA binds tightly with  SatB/atC, it may transition to an open conformation, which has decreased affinity  for sialic acid, and SatB/atC may reorient to expose a sugar binding site.	bind
10656	2	4319	5	NULL	NULL	0	NULL	SatB/atC	NULL		transition to	NULL	may			open conformation	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_73_10_6727_s_194	16177350	(B) When SatA binds tightly with  SatB/atC, it may transition to an open conformation, which has decreased affinity  for sialic acid, and SatB/atC may reorient to expose a sugar binding site.	bind
10662	3	4319	5	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_73_10_6727_s_194	16177350	(B) When SatA binds tightly with  SatB/atC, it may transition to an open conformation, which has decreased affinity  for sialic acid, and SatB/atC may reorient to expose a sugar binding site.	bind
10665	4	4319	5	NULL	NULL	0	NULL	statement 2	NULL		decreased affinity for	NULL				sialic acid	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_73_10_6727_s_194	16177350	(B) When SatA binds tightly with  SatB/atC, it may transition to an open conformation, which has decreased affinity  for sialic acid, and SatB/atC may reorient to expose a sugar binding site.	bind
10667	5	4319	5	10	NULL	0	NULL	SatB/atC			expose		may						sugar binding site		NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_10_6727_s_194	16177350	(B) When SatA binds tightly with  SatB/atC, it may transition to an open conformation, which has decreased affinity  for sialic acid, and SatB/atC may reorient to expose a sugar binding site.	bind
9876	1	4319	6	NULL	NULL	NULL	NULL	SatA	GP		bind		tightly			SatB/atC	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_10_6727_s_194	16177350	(B) When SatA binds tightly with  SatB/atC, it may transition to an open conformation, which has decreased affinity  for sialic acid, and SatB/atC may reorient to expose a sugar binding site.	bind
9877	2	4319	6	NULL	NULL	NULL	NULL	SatB/atC	GP		transition to		may			open conformation					NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_10_6727_s_194	16177350	(B) When SatA binds tightly with  SatB/atC, it may transition to an open conformation, which has decreased affinity  for sialic acid, and SatB/atC may reorient to expose a sugar binding site.	bind
9878	3	4319	6	NULL	NULL	NULL	NULL	SatA	GP	open conformation	has decreased affinity for					sialic acid	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_10_6727_s_194	16177350	(B) When SatA binds tightly with  SatB/atC, it may transition to an open conformation, which has decreased affinity  for sialic acid, and SatB/atC may reorient to expose a sugar binding site.	bind
9924	4	4319	6	NULL	NULL	NULL	NULL	SatB/atC	GP		expose		may						sugar binding site		NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_10_6727_s_194	16177350	(B) When SatA binds tightly with  SatB/atC, it may transition to an open conformation, which has decreased affinity  for sialic acid, and SatB/atC may reorient to expose a sugar binding site.	bind
12778	5	4319	6	NULL	NULL	NULL	NULL	statement 1	Process		lead to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_10_6727_s_194	16177350	(B) When SatA binds tightly with  SatB/atC, it may transition to an open conformation, which has decreased affinity  for sialic acid, and SatB/atC may reorient to expose a sugar binding site.	bind
10668	1	4320	5	NULL	NULL	0	NULL	phospho-LIS1 isoform	NULL		bind	NULL				MT bundles	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_9_3089_s_298	11940666	(b) When the distal zinc finger motif of CLIP-170 is mutated, the phospho-LIS1 isoform can no longer bind to MT bundles.	bind
10669	2	4320	5	10	NULL	0	NULL	CLIP-170		mutation of 	prevent			distal zinc finger motif		statement 1					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_3089_s_298	11940666	(b) When the distal zinc finger motif of CLIP-170 is mutated, the phospho-LIS1 isoform can no longer bind to MT bundles.	bind
9879	1	4320	6	NULL	NULL	NULL	NULL	phospho-LIS1 isoform	GP		bind					MT bundles	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_3089_s_298	11940666	(b) When the distal zinc finger motif of CLIP-170 is mutated, the phospho-LIS1 isoform can no longer bind to MT bundles.	bind
9880	2	4320	6	NULL	NULL	NULL	NULL	CLIP-170	GP	mutant	attenuates			distal zinc finger motif		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_3089_s_298	11940666	(b) When the distal zinc finger motif of CLIP-170 is mutated, the phospho-LIS1 isoform can no longer bind to MT bundles.	bind
10670	1	4321	5	NULL	NULL	0	NULL	BimL protein	NULL	wild-type	bind	NULL	tightly			Bcl-w	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_162_5_877_s_98	12952938	(B) Wild-type BimL protein and its BH3 peptide bind tightly to Bcl-w.	bind
10671	2	4321	5	NULL	NULL	0	NULL	BH3 peptide	NULL		bind	NULL	tightly			Bcl-w	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_162_5_877_s_98	12952938	(B) Wild-type BimL protein and its BH3 peptide bind tightly to Bcl-w.	bind
9881	1	4321	6	NULL	NULL	NULL	NULL	BimL protein	GP	wild type	bind		tightly			Bcl-w	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_162_5_877_s_98	12952938	(B) Wild-type BimL protein and its BH3 peptide bind tightly to Bcl-w.	bind
9882	2	4321	6	NULL	NULL	NULL	NULL	BH3 peptide	AminoAcid		bind		tightly			Bcl-w	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_162_5_877_s_98	12952938	(B) Wild-type BimL protein and its BH3 peptide bind tightly to Bcl-w.	bind
10676	1	4323	5	NULL	NULL	0	NULL	CLK	NULL		bind	NULL					NULL			per sequences	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_18_6935_s_222	10958689	(B) Yeast one-hybrid assays showing the binding of CLK and CYC to  per and  to upstream sequences.	bind
10677	2	4323	5	NULL	NULL	0	NULL	CYC	NULL		bind	NULL					NULL			per sequences	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_18_6935_s_222	10958689	(B) Yeast one-hybrid assays showing the binding of CLK and CYC to  per and  to upstream sequences.	bind
12657	1	4323	6	NULL	NULL	NULL	NULL	CLK	GP		bind						GP			per sequences	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_18_6935_s_222	10958689	(B) Yeast one-hybrid assays showing the binding of CLK and CYC to  per and  to upstream sequences.	bind
12658	2	4323	6	NULL	NULL	NULL	NULL	CYC	GP		bind						GP			per sequences	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_18_6935_s_222	10958689	(B) Yeast one-hybrid assays showing the binding of CLK and CYC to  per and  to upstream sequences.	bind
10680	1	4324	5	NULL	NULL	0	NULL	membrane pore complex	NULL		formed by	NULL				Sec61	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_108_5_591_s_32	11893330	(B) Yeast ribosome bound to the membrane pore complex formed by Sec61 (red).	bind
10681	2	4324	5	NULL	NULL	0	NULL	ribosome	NULL	yeast	bind	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_108_5_591_s_32	11893330	(B) Yeast ribosome bound to the membrane pore complex formed by Sec61 (red).	bind
9885	1	4324	6	NULL	NULL	NULL	NULL	Sec61	GP		form					membrane pore complex	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cell_108_5_591_s_32	11893330	(B) Yeast ribosome bound to the membrane pore complex formed by Sec61 (red).	bind
9886	2	4324	6	NULL	NULL	NULL	NULL	ribosome	CellComponent	yeast	bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_108_5_591_s_32	11893330	(B) Yeast ribosome bound to the membrane pore complex formed by Sec61 (red).	bind
10682	1	4325	5	NULL	NULL	0	NULL	DCAPS	NULL		bind	NULL				Axin	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_2_229_s_72	12711303	(B) Yeast two-hybrid assay for the binding of DCAPS to Axin,  Dfz2, and Dsh.	bind
10683	2	4325	5	NULL	NULL	0	NULL	DCAPS	NULL		bind	NULL				Dfz2	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_2_229_s_72	12711303	(B) Yeast two-hybrid assay for the binding of DCAPS to Axin,  Dfz2, and Dsh.	bind
10684	3	4325	5	NULL	NULL	0	NULL	DCAPS	NULL		bind	NULL				Dsh	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_2_229_s_72	12711303	(B) Yeast two-hybrid assay for the binding of DCAPS to Axin,  Dfz2, and Dsh.	bind
9887	1	4325	6	NULL	NULL	NULL	NULL	DCAPS	GP		bind					Axin	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_2_229_s_72	12711303	(B) Yeast two-hybrid assay for the binding of DCAPS to Axin,  Dfz2, and Dsh.	bind
9888	2	4325	6	NULL	NULL	NULL	NULL	DCAPS	GP		bind					Dfz2	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_2_229_s_72	12711303	(B) Yeast two-hybrid assay for the binding of DCAPS to Axin,  Dfz2, and Dsh.	bind
9889	3	4325	6	NULL	NULL	NULL	NULL	DCAPS	GP		bind					Dsh	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_2_229_s_72	12711303	(B) Yeast two-hybrid assay for the binding of DCAPS to Axin,  Dfz2, and Dsh.	bind
10685	1	4327	5	10	NULL	0	NULL	rootletin fragments			derived from								rod domain		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_3_431_s_184	12427867	(B) Yeast two-hybrid assays show homotypic binding between rootletin fragments derived from the rod domain.	bind
54262	2	4327	5	10	NULL	0	NULL	rootletin fragments			bind		homotypically			rootletin fragments					NULL		0	NULL	NULL	NULL	gw60_cellbiol_159_3_431_s_184	12427867	(B) Yeast two-hybrid assays show homotypic binding between rootletin fragments derived from the rod domain.	bind
12660	1	4327	6	NULL	NULL	NULL	NULL	rootletin fragments	GP		are derived from								rod domain		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_3_431_s_184	12427867	(B) Yeast two-hybrid assays show homotypic binding between rootletin fragments derived from the rod domain.	bind
41326	2	4327	6	NULL	NULL	NULL	NULL	rootletin fragments	GP		bind		homotypically			rootletin fragments	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_3_431_s_184	12427867	(B) Yeast two-hybrid assays show homotypic binding between rootletin fragments derived from the rod domain.	bind
10692	1	4328	5	NULL	NULL	0	NULL		NULL	mutant	bind	NULL		pericentrin domain		GCP2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_8_3642_s_118	15146056	(B) Yeast two-hybrid data showing significantly  reduced binding of mutant pericentrin domain for GCP2 and GCP3.	bind
10693	2	4328	5	NULL	NULL	0	NULL		NULL	mutant	bind	NULL		pericentrin domain		GCP3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_8_3642_s_118	15146056	(B) Yeast two-hybrid data showing significantly  reduced binding of mutant pericentrin domain for GCP2 and GCP3.	bind
12662	1	4328	6	NULL	NULL	NULL	NULL			mutant	bind			pericentrin domain		GCP2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_8_3642_s_118	15146056	(B) Yeast two-hybrid data showing significantly  reduced binding of mutant pericentrin domain for GCP2 and GCP3.	bind
12663	2	4328	6	NULL	NULL	NULL	NULL			mutant	bind			pericentrin domain		GCP3	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_8_3642_s_118	15146056	(B) Yeast two-hybrid data showing significantly  reduced binding of mutant pericentrin domain for GCP2 and GCP3.	bind
10705	1	4330	5	NULL	NULL	0	NULL	YY1	NULL		bind	NULL					NULL			SR3	NULL		0	NULL	NULL	NULL	gw70_development_131_19_4709_s_208	15329343	(B) YY1 binds to SR3.	bind
9904	1	4330	6	NULL	NULL	NULL	NULL	YY1	GP		bind									SR3	NULL		NULL	NULL	NULL	NULL	gw70_development_131_19_4709_s_208	15329343	(B) YY1 binds to SR3.	bind
10706	1	4331	5	NULL	NULL	0	NULL	ZEN-4	NULL		bind	NULL		E502K		CYK-4	NULL		S15L		NULL		0	NULL	NULL	NULL	gw60_devcell_2_1_41_s_138	11782313	(B) ZEN-4(E502K) binds to CYK-4(S15L).	bind
9905	1	4331	6	NULL	NULL	NULL	NULL	ZEN-4	GP		bind			E502K		CYK-4	GP		S15L		NULL		NULL	NULL	NULL	NULL	gw60_devcell_2_1_41_s_138	11782313	(B) ZEN-4(E502K) binds to CYK-4(S15L).	bind
10707	1	4332	5	NULL	NULL	0	NULL	ZO-1	NULL		bind	NULL	directly	PDZ domains		ARVCF	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_12_5503_s_107	15456900	(B) ZO-1 PDZ domains bind directly to ARVCF in blot overlays.	bind
9906	1	4332	6	NULL	NULL	NULL	NULL	ZO-1	GP		bind		directly	PDZ domain		ARVCF	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_12_5503_s_107	15456900	(B) ZO-1 PDZ domains bind directly to ARVCF in blot overlays.	bind
10708	1	4333	5	10	NULL	0	NULL	[125] adrenomedullin	NULL	rat	bind	NULL				CHO-K1 cell membranes	NULL				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1539_1_131_s_73	11389975	(B) [125]Rat adrenomedullin binding to CHO-K1 cell membranes was assayed.	bind
9907	1	4333	6	NULL	NULL	NULL	NULL	[125] adrenomedullin	AminoAcid	rat	bind					CHO-K1 cell membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1539_1_131_s_73	11389975	(B) [125]Rat adrenomedullin binding to CHO-K1 cell membranes was assayed.	bind
10709	1	4335	5	NULL	NULL	0	NULL	HEK-293 cell membranes	NULL		express	NULL				D2R	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_38_2_291_s_175	12718862	(B) [35]GTP S binding to HEK-293 cell membranes expressing D2R was determined after stimulation with dopamine.	bind
10710	2	4335	5	10	NULL	0	NULL	GTP S			bind					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_neuron_38_2_291_s_175	12718862	(B) [35]GTP S binding to HEK-293 cell membranes expressing D2R was determined after stimulation with dopamine.	bind
10711	3	4335	5	NULL	NULL	0	NULL	dopamine	NULL	stimulation by	is required for	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuron_38_2_291_s_175	12718862	(B) [35]GTP S binding to HEK-293 cell membranes expressing D2R was determined after stimulation with dopamine.	bind
9908	1	4335	6	NULL	NULL	NULL	NULL	HEK-293 cell membranes	CellComponent		express					D2R	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_38_2_291_s_175	12718862	(B) [35]GTP S binding to HEK-293 cell membranes expressing D2R was determined after stimulation with dopamine.	bind
9909	2	4335	6	NULL	NULL	NULL	NULL	GTP S	Chemical		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_38_2_291_s_175	12718862	(B) [35]GTP S binding to HEK-293 cell membranes expressing D2R was determined after stimulation with dopamine.	bind
9910	3	4335	6	NULL	NULL	NULL	NULL	statement 2	Process		after stimulation with					dopamine	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_neuron_38_2_291_s_175	12718862	(B) [35]GTP S binding to HEK-293 cell membranes expressing D2R was determined after stimulation with dopamine.	bind
10713	1	4339	5	NULL	NULL	0	NULL	ZEB-1/deltaEF1	NULL		bind	NULL				R-Smads	NULL	activated			NULL		0	NULL	NULL	NULL	gw60_embo_22_10_2443_s_29	12743038	(B, C and D) ZEB-1/deltaEF1 and ZEB-2/SIP1 bind to activated R-Smads.	bind
10714	2	4339	5	NULL	NULL	0	NULL	ZEB-2/SIP1	NULL		bind	NULL				R-Smads	NULL	activated			NULL		0	NULL	NULL	NULL	gw60_embo_22_10_2443_s_29	12743038	(B, C and D) ZEB-1/deltaEF1 and ZEB-2/SIP1 bind to activated R-Smads.	bind
9911	1	4339	6	NULL	NULL	NULL	NULL	ZEB-1/deltaEF1	GP		bind					R-Smads	GP	activated			NULL		NULL	NULL	NULL	NULL	gw60_embo_22_10_2443_s_29	12743038	(B, C and D) ZEB-1/deltaEF1 and ZEB-2/SIP1 bind to activated R-Smads.	bind
9912	2	4339	6	NULL	NULL	NULL	NULL	ZEB-2/SIP1	GP		bind					R-Smads	GP	activated			NULL		NULL	NULL	NULL	NULL	gw60_embo_22_10_2443_s_29	12743038	(B, C and D) ZEB-1/deltaEF1 and ZEB-2/SIP1 bind to activated R-Smads.	bind
10715	1	4340	5	NULL	NULL	0	NULL	NF-kappaB	NULL		bind	NULL				DNA	NULL				NULL	in lymphocytes exposed to PMA/ionomycin	0	NULL	NULL	NULL	gw60_brjpharmacol_137_6_761_s_177	12411406	(B, C) Identical concentrations of PHE and BZD reduce the DNA binding activity of NF-kappaB and AP-1 in lymphocytes exposed 1 or 2 h to PMA/ionomycin.	bind
10716	2	4340	5	NULL	NULL	0	NULL	AP-1	NULL		bind	NULL				DNA	NULL				NULL	in lymphocytes exposed to PMA/ionomycin	0	NULL	NULL	NULL	gw60_brjpharmacol_137_6_761_s_177	12411406	(B, C) Identical concentrations of PHE and BZD reduce the DNA binding activity of NF-kappaB and AP-1 in lymphocytes exposed 1 or 2 h to PMA/ionomycin.	bind
10717	3	4340	5	NULL	NULL	0	NULL	PHE	NULL		reduce	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_137_6_761_s_177	12411406	(B, C) Identical concentrations of PHE and BZD reduce the DNA binding activity of NF-kappaB and AP-1 in lymphocytes exposed 1 or 2 h to PMA/ionomycin.	bind
10718	4	4340	5	NULL	NULL	0	NULL	PHE	NULL		reduce	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_137_6_761_s_177	12411406	(B, C) Identical concentrations of PHE and BZD reduce the DNA binding activity of NF-kappaB and AP-1 in lymphocytes exposed 1 or 2 h to PMA/ionomycin.	bind
10719	5	4340	5	NULL	NULL	0	NULL	BZD	NULL		reduce	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_137_6_761_s_177	12411406	(B, C) Identical concentrations of PHE and BZD reduce the DNA binding activity of NF-kappaB and AP-1 in lymphocytes exposed 1 or 2 h to PMA/ionomycin.	bind
10720	6	4340	5	NULL	NULL	0	NULL	BZD	NULL		reduce	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_137_6_761_s_177	12411406	(B, C) Identical concentrations of PHE and BZD reduce the DNA binding activity of NF-kappaB and AP-1 in lymphocytes exposed 1 or 2 h to PMA/ionomycin.	bind
9913	1	4340	6	NULL	NULL	NULL	NULL	NF-kappaB	GP		bind					DNA	NucleicAcid				NULL	lymphocytes exposed to PMA/ionomycin	NULL	NULL	NULL	NULL	gw60_brjpharmacol_137_6_761_s_177	12411406	(B, C) Identical concentrations of PHE and BZD reduce the DNA binding activity of NF-kappaB and AP-1 in lymphocytes exposed 1 or 2 h to PMA/ionomycin.	bind
9914	2	4340	6	NULL	NULL	NULL	NULL	AP-1	GP		bind					DNA	NucleicAcid				NULL	lymphocytes exposed to PMA/ionomycin	NULL	NULL	NULL	NULL	gw60_brjpharmacol_137_6_761_s_177	12411406	(B, C) Identical concentrations of PHE and BZD reduce the DNA binding activity of NF-kappaB and AP-1 in lymphocytes exposed 1 or 2 h to PMA/ionomycin.	bind
9915	3	4340	6	NULL	NULL	NULL	NULL	PHE			reduce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_137_6_761_s_177	12411406	(B, C) Identical concentrations of PHE and BZD reduce the DNA binding activity of NF-kappaB and AP-1 in lymphocytes exposed 1 or 2 h to PMA/ionomycin.	bind
9916	4	4340	6	NULL	NULL	NULL	NULL	PHE			reduce					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_137_6_761_s_177	12411406	(B, C) Identical concentrations of PHE and BZD reduce the DNA binding activity of NF-kappaB and AP-1 in lymphocytes exposed 1 or 2 h to PMA/ionomycin.	bind
9917	5	4340	6	NULL	NULL	NULL	NULL	BZD	GP		reduce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_137_6_761_s_177	12411406	(B, C) Identical concentrations of PHE and BZD reduce the DNA binding activity of NF-kappaB and AP-1 in lymphocytes exposed 1 or 2 h to PMA/ionomycin.	bind
9918	6	4340	6	NULL	NULL	NULL	NULL	BZD	GP		reduce					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_137_6_761_s_177	12411406	(B, C) Identical concentrations of PHE and BZD reduce the DNA binding activity of NF-kappaB and AP-1 in lymphocytes exposed 1 or 2 h to PMA/ionomycin.	bind
10721	1	4341	5	NULL	NULL	0	NULL	LacI-GFP	NULL		bind	NULL					NULL			 lac operator	NULL	in spo0J+ (strain DCL696) cells	NULL	NULL	NULL	NULL	gw70_jbacteriol_185_4_1326_s_163	12562803	(B, C) Position of sister origin regions (359 degrees ) visualized  with LacI-GFP bound to  lac operator arrays in  spo0J+ (strain DCL696) and  spo0J mutant (strain DCL705) cells.	bind
10722	2	4341	5	NULL	NULL	0	NULL	LacI-GFP	NULL		bind	NULL					NULL			lac operator	NULL	in spo0J mutant (strain DCL705) cells	0	NULL	NULL	NULL	gw70_jbacteriol_185_4_1326_s_163	12562803	(B, C) Position of sister origin regions (359 degrees ) visualized  with LacI-GFP bound to  lac operator arrays in  spo0J+ (strain DCL696) and  spo0J mutant (strain DCL705) cells.	bind
12779	1	4341	6	NULL	NULL	NULL	NULL	LacI-GFP			bind						NucleicAcid			lac operator	NULL	spo0J+ (strain DCL696) cells)	NULL	NULL	NULL	NULL	gw70_jbacteriol_185_4_1326_s_163	12562803	(B, C) Position of sister origin regions (359 degrees ) visualized  with LacI-GFP bound to  lac operator arrays in  spo0J+ (strain DCL696) and  spo0J mutant (strain DCL705) cells.	bind
12780	2	4341	6	NULL	NULL	NULL	NULL	LacI-GFP			bind						NucleicAcid			lac operator	NULL	spo0J mutant (strain DCL705) cells	NULL	NULL	NULL	NULL	gw70_jbacteriol_185_4_1326_s_163	12562803	(B, C) Position of sister origin regions (359 degrees ) visualized  with LacI-GFP bound to  lac operator arrays in  spo0J+ (strain DCL696) and  spo0J mutant (strain DCL705) cells.	bind
10723	1	4343	5	NULL	NULL	0	NULL	EGFR	NULL		does not bind	NULL		tryptic domains		F-actin	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_312_4_930_s_135	14651960	(B,C)  Tryptic domains of the EGFR do not bind F-actin.	bind
9919	1	4343	6	NULL	NULL	NULL	NULL	EGFR	GP		does not bind			tryptic domains		F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_312_4_930_s_135	14651960	(B,C)  Tryptic domains of the EGFR do not bind F-actin.	bind
10724	1	4345	5	NULL	NULL	0	NULL		NULL		bind	NULL		envelope domains		HBcAg protein	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_319_3_959_s_123	15184075	(B,C) Binding of envelope domains and HBcAg protein.	bind
9920	1	4345	6	NULL	NULL	NULL	NULL				bind			envelop domains		HBcAg protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_319_3_959_s_123	15184075	(B,C) Binding of envelope domains and HBcAg protein.	bind
10725	1	4346	5	10	NULL	0	NULL	P30-34			bind					DCs					NULL		NULL	NULL	NULL	NULL	gw70_febslett_579_7_1658_s_75	15757657	(B-D) FACS analysis of  P30-34 binding to DCs. (B) DCs were incubated with 3  M of the indicated proteins  for 1.5 h. DCs were then incubated with a rabbit anti-bvPLA2 serum and with a phycoerythrin anti-rabbit IgG antibody.	bind
9942	1	4346	6	NULL	NULL	NULL	NULL	P30-34			bind					DCs	Cell				NULL		NULL	NULL	NULL	NULL	gw70_febslett_579_7_1658_s_75	15757657	(B-D) FACS analysis of  P30-34 binding to DCs. (B) DCs were incubated with 3  M of the indicated proteins  for 1.5 h. DCs were then incubated with a rabbit anti-bvPLA2 serum and with a phycoerythrin anti-rabbit IgG antibody.	bind
10726	1	4348	5	NULL	NULL	0	NULL	Xlim-1	NULL		bind	NULL				cerberus	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_devbiol_257_1_190_s_296	12710967	(B-D) Xlim-1, Mix.1, Siamois, and Xotx2 bind to the  cerberus promoter.	bind
10727	2	4348	5	NULL	NULL	0	NULL	Mix.1	NULL		bind	NULL				cerberus	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_devbiol_257_1_190_s_296	12710967	(B-D) Xlim-1, Mix.1, Siamois, and Xotx2 bind to the  cerberus promoter.	bind
10728	3	4348	5	NULL	NULL	0	NULL	Siamois	NULL		bind	NULL				cerberus	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_devbiol_257_1_190_s_296	12710967	(B-D) Xlim-1, Mix.1, Siamois, and Xotx2 bind to the  cerberus promoter.	bind
10729	4	4348	5	NULL	NULL	0	NULL	Xotx2	NULL		bind	NULL				cerberus	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_devbiol_257_1_190_s_296	12710967	(B-D) Xlim-1, Mix.1, Siamois, and Xotx2 bind to the  cerberus promoter.	bind
9943	1	4348	6	NULL	NULL	NULL	NULL	Xlim-1	GP		bind					cerberus	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_devbiol_257_1_190_s_296	12710967	(B-D) Xlim-1, Mix.1, Siamois, and Xotx2 bind to the  cerberus promoter.	bind
9944	2	4348	6	NULL	NULL	NULL	NULL	Mix.1	GP		bind					cerberus	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_devbiol_257_1_190_s_296	12710967	(B-D) Xlim-1, Mix.1, Siamois, and Xotx2 bind to the  cerberus promoter.	bind
9945	3	4348	6	NULL	NULL	NULL	NULL	Siamois	GP		bind					cerberus	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_devbiol_257_1_190_s_296	12710967	(B-D) Xlim-1, Mix.1, Siamois, and Xotx2 bind to the  cerberus promoter.	bind
9946	4	4348	6	NULL	NULL	NULL	NULL	Xotx2	GP		bind					cerberus	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_devbiol_257_1_190_s_296	12710967	(B-D) Xlim-1, Mix.1, Siamois, and Xotx2 bind to the  cerberus promoter.	bind
11444	1	4349	5	10	NULL	0	NULL	neuropilin-2 ectodomain-Fc		soluble	bind					neuropilin-2					NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_6_1283_s_25	9883722	(B-G) Binding of neuropilins in  trans was observed through binding of a soluble neuropilin-2 ectodomain-Fc fusion protein to neuropilin-2(a0) expressed in COS cells (B and E), neuropilin-1 expressed in COS cells (C and F), or control COS cells (D and G) in the absence (B-D) or presence (E-G) of Sema E (similar results were obtained with Sema IV (data not shown)).	bind
11445	2	4349	5	10	NULL	0	NULL	neuropilin-2 ectodomain-Fc		soluble	bind					neuropilin-1					NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_6_1283_s_25	9883722	(B-G) Binding of neuropilins in  trans was observed through binding of a soluble neuropilin-2 ectodomain-Fc fusion protein to neuropilin-2(a0) expressed in COS cells (B and E), neuropilin-1 expressed in COS cells (C and F), or control COS cells (D and G) in the absence (B-D) or presence (E-G) of Sema E (similar results were obtained with Sema IV (data not shown)).	bind
44437	3	4349	5	10	NULL	0	NULL	neuropilin-2	NULL		is expressed in	NULL				COS cells	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_6_1283_s_25	9883722	(B-G) Binding of neuropilins in  trans was observed through binding of a soluble neuropilin-2 ectodomain-Fc fusion protein to neuropilin-2(a0) expressed in COS cells (B and E), neuropilin-1 expressed in COS cells (C and F), or control COS cells (D and G) in the absence (B-D) or presence (E-G) of Sema E (similar results were obtained with Sema IV (data not shown)).	bind
44438	4	4349	5	10	NULL	0	NULL	neuropilin-1 	NULL		is expressed in	NULL				COS cells	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_21_6_1283_s_25	9883722	(B-G) Binding of neuropilins in  trans was observed through binding of a soluble neuropilin-2 ectodomain-Fc fusion protein to neuropilin-2(a0) expressed in COS cells (B and E), neuropilin-1 expressed in COS cells (C and F), or control COS cells (D and G) in the absence (B-D) or presence (E-G) of Sema E (similar results were obtained with Sema IV (data not shown)).	bind
57787	5	4349	5	10	NULL	0	NULL	\tneuropilin-2 ectodomain-Fc			is a type of					fusion protein					NULL		0	NULL	NULL	NULL	gw60_neuron_21_6_1283_s_25	9883722	(B-G) Binding of neuropilins in  trans was observed through binding of a soluble neuropilin-2 ectodomain-Fc fusion protein to neuropilin-2(a0) expressed in COS cells (B and E), neuropilin-1 expressed in COS cells (C and F), or control COS cells (D and G) in the absence (B-D) or presence (E-G) of Sema E (similar results were obtained with Sema IV (data not shown)).	bind
9947	1	4349	6	NULL	NULL	NULL	NULL	neuropilin-2 ectodomain-Fc 	GP	soluble	bind					neuropilin-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_6_1283_s_25	9883722	(B-G) Binding of neuropilins in  trans was observed through binding of a soluble neuropilin-2 ectodomain-Fc fusion protein to neuropilin-2(a0) expressed in COS cells (B and E), neuropilin-1 expressed in COS cells (C and F), or control COS cells (D and G) in the absence (B-D) or presence (E-G) of Sema E (similar results were obtained with Sema IV (data not shown)).	bind
9948	2	4349	6	NULL	NULL	NULL	NULL	neuropilin-2 ectodomain-Fc	GP	soluble	bind					neuropilin-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_6_1283_s_25	9883722	(B-G) Binding of neuropilins in  trans was observed through binding of a soluble neuropilin-2 ectodomain-Fc fusion protein to neuropilin-2(a0) expressed in COS cells (B and E), neuropilin-1 expressed in COS cells (C and F), or control COS cells (D and G) in the absence (B-D) or presence (E-G) of Sema E (similar results were obtained with Sema IV (data not shown)).	bind
9949	3	4349	6	NULL	NULL	NULL	NULL	neuropilin-1	GP		is expressed in					COS cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_6_1283_s_25	9883722	(B-G) Binding of neuropilins in  trans was observed through binding of a soluble neuropilin-2 ectodomain-Fc fusion protein to neuropilin-2(a0) expressed in COS cells (B and E), neuropilin-1 expressed in COS cells (C and F), or control COS cells (D and G) in the absence (B-D) or presence (E-G) of Sema E (similar results were obtained with Sema IV (data not shown)).	bind
57788	4	4349	6	NULL	NULL	NULL	NULL	neuropilin-2	GP		is expressed in					COS cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_6_1283_s_25	9883722	(B-G) Binding of neuropilins in  trans was observed through binding of a soluble neuropilin-2 ectodomain-Fc fusion protein to neuropilin-2(a0) expressed in COS cells (B and E), neuropilin-1 expressed in COS cells (C and F), or control COS cells (D and G) in the absence (B-D) or presence (E-G) of Sema E (similar results were obtained with Sema IV (data not shown)).	bind
57789	5	4349	6	NULL	NULL	NULL	NULL	neuropilin-2 ectodomain-Fc	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_6_1283_s_25	9883722	(B-G) Binding of neuropilins in  trans was observed through binding of a soluble neuropilin-2 ectodomain-Fc fusion protein to neuropilin-2(a0) expressed in COS cells (B and E), neuropilin-1 expressed in COS cells (C and F), or control COS cells (D and G) in the absence (B-D) or presence (E-G) of Sema E (similar results were obtained with Sema IV (data not shown)).	bind
10754	1	4350	5	10	NULL	0	NULL	Sema IV-AP fusion	NULL	full length	bind	NULL				neuropilin-2	NULL	truncated forms of			NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_6_1283_s_129	9883722	(B-J) Binding of AP fusions of full length and truncated versions of Sema IV to truncated forms of neuropilin-2(a0).	bind
10755	2	4350	5	10	NULL	0	NULL	Sema IV-AP fusion		 truncated 	bind					neuropilin-2		truncated forms of			NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_6_1283_s_129	9883722	(B-J) Binding of AP fusions of full length and truncated versions of Sema IV to truncated forms of neuropilin-2(a0).	bind
9950	1	4350	6	NULL	NULL	NULL	NULL	Sema IV-AP fusion	GP	full length	bind					neuropilin-2	GP	truncated forms of 			NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_6_1283_s_129	9883722	(B-J) Binding of AP fusions of full length and truncated versions of Sema IV to truncated forms of neuropilin-2(a0).	bind
9951	2	4350	6	NULL	NULL	NULL	NULL	Sema IV-AP fusion	GP	truncated 	bind					neuropilin-2	GP	truncated forms of			NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_6_1283_s_129	9883722	(B-J) Binding of AP fusions of full length and truncated versions of Sema IV to truncated forms of neuropilin-2(a0).	bind
10753	1	4352	5	NULL	NULL	0	NULL	RNA	NULL		bind	NULL				BBR	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_5_2_395_s_58	10882080	(b-m) RNA binding to the BBR (b-g) and DNA binding to the DNA target sequence ATCTAATCCC (h-m) of the wild-type BCD HD (HDwt) and single amino acid replacement mutants.	bind
11446	2	4352	5	NULL	NULL	0	NULL	DNA	NULL		bind	NULL				BCD	NULL	wild-type		DNA target sequence ATCTAATCCC in HD	NULL		0	NULL	NULL	NULL	gw60_molcell_5_2_395_s_58	10882080	(b-m) RNA binding to the BBR (b-g) and DNA binding to the DNA target sequence ATCTAATCCC (h-m) of the wild-type BCD HD (HDwt) and single amino acid replacement mutants.	bind
9952	1	4352	6	NULL	NULL	NULL	NULL	RNA	NucleicAcid		bind					BBR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_2_395_s_58	10882080	(b-m) RNA binding to the BBR (b-g) and DNA binding to the DNA target sequence ATCTAATCCC (h-m) of the wild-type BCD HD (HDwt) and single amino acid replacement mutants.	bind
9953	2	4352	6	NULL	NULL	NULL	NULL	DNA	NucleicAcid		bind					BCD	NucleicAcid	wild type		DNA target sequence ATCTAATCCC in HD	NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_2_395_s_58	10882080	(b-m) RNA binding to the BBR (b-g) and DNA binding to the DNA target sequence ATCTAATCCC (h-m) of the wild-type BCD HD (HDwt) and single amino acid replacement mutants.	bind
11448	1	4354	5	NULL	NULL	0	NULL	Gcn4p	NULL		bind	NULL					NULL			TATA region	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_8_3135_s_72	16581788	(Because the UAS and TATA elements are separated by <200 bp and the sheared chromatin fragments are  500 bp, most fragments containing the TATA element also contain the UAS, likely accounting for the apparent binding of Gcn4p to the TATA region.)	bind
9954	1	4354	6	NULL	NULL	NULL	NULL	Gcn4p	GP		bind						NucleicAcid			TATA box	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_8_3135_s_72	16581788	(Because the UAS and TATA elements are separated by <200 bp and the sheared chromatin fragments are  500 bp, most fragments containing the TATA element also contain the UAS, likely accounting for the apparent binding of Gcn4p to the TATA region.)	bind
10756	1	4355	5	NULL	NULL	0	NULL	CcpC	NULL		bind	NULL				 ccpC	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_1_179_s_234	16352834	(Binding of CcpC to the  ccpC promoter relies on a Box I sequence only and is not affected by citrate [ ]).	bind
10757	2	4355	5	NULL	NULL	0	NULL	statement 1	NULL		relies on	NULL	only				NULL			Box I sequence	NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_1_179_s_234	16352834	(Binding of CcpC to the  ccpC promoter relies on a Box I sequence only and is not affected by citrate [ ]).	bind
10758	3	4355	5	NULL	NULL	0	NULL	statement 1	NULL		is not affected by	NULL				citrate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_1_179_s_234	16352834	(Binding of CcpC to the  ccpC promoter relies on a Box I sequence only and is not affected by citrate [ ]).	bind
9955	1	4355	6	NULL	NULL	NULL	NULL	CcpC	GP		bind					ccpC	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_1_179_s_234	16352834	(Binding of CcpC to the  ccpC promoter relies on a Box I sequence only and is not affected by citrate [ ]).	bind
9956	2	4355	6	NULL	NULL	NULL	NULL	statement 1	Process		is not affected by					citrate	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_1_179_s_234	16352834	(Binding of CcpC to the  ccpC promoter relies on a Box I sequence only and is not affected by citrate [ ]).	bind
9957	3	4355	6	NULL	NULL	NULL	NULL	statement 1	Process		is dependent on		only				NucleicAcid			Box I sequence	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_1_179_s_234	16352834	(Binding of CcpC to the  ccpC promoter relies on a Box I sequence only and is not affected by citrate [ ]).	bind
10759	1	4358	5	NULL	NULL	0	NULL	I-mfa	NULL		bind	NULL				Axin	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_271	12192039	(Bottom panel) I-mfa binding to Axin does not affect the binding of GSK-3beta, and the activation of JNK is decreased.	bind
10760	2	4358	5	NULL	NULL	0	NULL	statement 1	NULL		does not affect	NULL				GSK-3beta	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_271	12192039	(Bottom panel) I-mfa binding to Axin does not affect the binding of GSK-3beta, and the activation of JNK is decreased.	bind
10837	3	4358	5	NULL	NULL	0	NULL	statement 1	NULL		decrease	NULL				JNK	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_271	12192039	(Bottom panel) I-mfa binding to Axin does not affect the binding of GSK-3beta, and the activation of JNK is decreased.	bind
9958	1	4358	6	NULL	NULL	NULL	NULL	 I-mfa	GP		bind					Axin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_271	12192039	(Bottom panel) I-mfa binding to Axin does not affect the binding of GSK-3beta, and the activation of JNK is decreased.	bind
9959	2	4358	6	NULL	NULL	NULL	NULL	statement 1	Process		does not affect					GSK-3beta	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_271	12192039	(Bottom panel) I-mfa binding to Axin does not affect the binding of GSK-3beta, and the activation of JNK is decreased.	bind
12676	3	4358	6	NULL	NULL	NULL	NULL	statement 1	Process		decrease					JNK	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_271	12192039	(Bottom panel) I-mfa binding to Axin does not affect the binding of GSK-3beta, and the activation of JNK is decreased.	bind
10838	1	4361	5	NULL	NULL	0	NULL	HVEM:Fc	NULL		bind	NULL				II-23 cells	NULL	activated			NULL		0	NULL	NULL	NULL	gw60_immunity_8_1_21_s_65	9462508	(Bottom) dose dependence of LT  competition for HVEM:Fc binding to activated II-23 cells as determined by flow cytofluorometry.	bind
10839	2	4361	5	NULL	NULL	0	NULL	LT	NULL		bind	NULL				II-23 cells	NULL	activated			NULL		0	NULL	NULL	NULL	gw60_immunity_8_1_21_s_65	9462508	(Bottom) dose dependence of LT  competition for HVEM:Fc binding to activated II-23 cells as determined by flow cytofluorometry.	bind
10840	3	4361	5	NULL	NULL	0	NULL	statement 2	NULL		compete with	NULL	dose dependently			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_immunity_8_1_21_s_65	9462508	(Bottom) dose dependence of LT  competition for HVEM:Fc binding to activated II-23 cells as determined by flow cytofluorometry.	bind
9960	1	4361	6	NULL	NULL	NULL	NULL	HVEM:Fc	GP		bind					II-23 cells	Cell	activated			NULL		NULL	NULL	NULL	NULL	gw60_immunity_8_1_21_s_65	9462508	(Bottom) dose dependence of LT  competition for HVEM:Fc binding to activated II-23 cells as determined by flow cytofluorometry.	bind
9961	2	4361	6	NULL	NULL	NULL	NULL	LT	GP		bind					II-23 cells	Cell	activated			NULL		NULL	NULL	NULL	NULL	gw60_immunity_8_1_21_s_65	9462508	(Bottom) dose dependence of LT  competition for HVEM:Fc binding to activated II-23 cells as determined by flow cytofluorometry.	bind
9962	3	4361	6	NULL	NULL	NULL	NULL	statement 1	Process		competes		dose dependently			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_8_1_21_s_65	9462508	(Bottom) dose dependence of LT  competition for HVEM:Fc binding to activated II-23 cells as determined by flow cytofluorometry.	bind
10841	1	4362	5	NULL	NULL	0	NULL	LT R:Fc	NULL		inhibit	NULL	dose dependently			HVEM:Fc	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_immunity_8_1_21_s_59	9462508	(Bottom) dose-dependent inhibition of HVEM:Fc binding by LT R:Fc.	bind
9963	1	4362	6	NULL	NULL	NULL	NULL	LT R:Fc	GP		inhibits		dose dependently			HVEM:Fc	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_immunity_8_1_21_s_59	9462508	(Bottom) dose-dependent inhibition of HVEM:Fc binding by LT R:Fc.	bind
10842	1	4364	5	NULL	NULL	0	NULL	eIF2beta	NULL		bind	NULL				p97	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_25_17_4008_s_76	16932749	(Bottom) eIF2beta bound to p97 was quantified with a densitometer.	bind
9964	1	4364	6	NULL	NULL	NULL	NULL	eIF2beta	GP		bind					p97	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_17_4008_s_76	16932749	(Bottom) eIF2beta bound to p97 was quantified with a densitometer.	bind
10843	1	4365	5	NULL	NULL	0	NULL	S. pneumoniae cells	NULL	FITC-labeled	adhere to	NULL				CHO-ICAM-1 cells	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_74_2_830_s_121	16428725	(Bottom) Few FITC-labeled  S. pneumoniae cells (green) adhere to CHO-ICAM-1 cells.	bind
9965	1	4365	6	NULL	NULL	NULL	NULL	S. pneumoniae cells	Cell	FITC labeled	adhere to					CHO-ICAM-1 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_74_2_830_s_121	16428725	(Bottom) Few FITC-labeled  S. pneumoniae cells (green) adhere to CHO-ICAM-1 cells.	bind
10876	2	4366	5	10	NULL	0	NULL	statement 1			bind					PP1					NULL		NULL	NULL	NULL	NULL	gw60_cell_105_1_115_s_84	11301007	(Bottom) Fluctuations  in the simulation of three states of  the enzyme: (i) The inactive and assembled structure (including  SH2 and SH3) bound to PP1 (blue), (ii) the isolated  kinase domain in the absence of the  SH3 and SH2 domains bound to PP1  (green), and (iii) the isolated kinase domain in the  absence of PP1 (red).	bind
10877	1	4366	5	10	NULL	0	NULL	assembled structure			include								SH2 and SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_105_1_115_s_84	11301007	(Bottom) Fluctuations  in the simulation of three states of  the enzyme: (i) The inactive and assembled structure (including  SH2 and SH3) bound to PP1 (blue), (ii) the isolated  kinase domain in the absence of the  SH3 and SH2 domains bound to PP1  (green), and (iii) the isolated kinase domain in the  absence of PP1 (red).	bind
10878	3	4366	5	10	NULL	0	NULL			isolated	bind			kinase domain		PP1					NULL		NULL	NULL	NULL	NULL	gw60_cell_105_1_115_s_84	11301007	(Bottom) Fluctuations  in the simulation of three states of  the enzyme: (i) The inactive and assembled structure (including  SH2 and SH3) bound to PP1 (blue), (ii) the isolated  kinase domain in the absence of the  SH3 and SH2 domains bound to PP1  (green), and (iii) the isolated kinase domain in the  absence of PP1 (red).	bind
10879	4	4366	5	10	NULL	0	NULL	statement 3			in the absence of								SH2 domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_105_1_115_s_84	11301007	(Bottom) Fluctuations  in the simulation of three states of  the enzyme: (i) The inactive and assembled structure (including  SH2 and SH3) bound to PP1 (blue), (ii) the isolated  kinase domain in the absence of the  SH3 and SH2 domains bound to PP1  (green), and (iii) the isolated kinase domain in the  absence of PP1 (red).	bind
10880	5	4366	5	10	NULL	0	NULL	statement 3			in the absence of								SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_105_1_115_s_84	11301007	(Bottom) Fluctuations  in the simulation of three states of  the enzyme: (i) The inactive and assembled structure (including  SH2 and SH3) bound to PP1 (blue), (ii) the isolated  kinase domain in the absence of the  SH3 and SH2 domains bound to PP1  (green), and (iii) the isolated kinase domain in the  absence of PP1 (red).	bind
9966	1	4366	6	10	NULL	0	NULL	assembled structure			include								SH2 and SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_105_1_115_s_84	11301007	(Bottom) Fluctuations  in the simulation of three states of  the enzyme: (i) The inactive and assembled structure (including  SH2 and SH3) bound to PP1 (blue), (ii) the isolated  kinase domain in the absence of the  SH3 and SH2 domains bound to PP1  (green), and (iii) the isolated kinase domain in the  absence of PP1 (red).	bind
9967	2	4366	6	NULL	NULL	NULL	NULL	statement 1	Process		bind					PP1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_105_1_115_s_84	11301007	(Bottom) Fluctuations  in the simulation of three states of  the enzyme: (i) The inactive and assembled structure (including  SH2 and SH3) bound to PP1 (blue), (ii) the isolated  kinase domain in the absence of the  SH3 and SH2 domains bound to PP1  (green), and (iii) the isolated kinase domain in the  absence of PP1 (red).	bind
9968	3	4366	6	NULL	NULL	NULL	NULL			isolated	bind			kinase domain		PP1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_105_1_115_s_84	11301007	(Bottom) Fluctuations  in the simulation of three states of  the enzyme: (i) The inactive and assembled structure (including  SH2 and SH3) bound to PP1 (blue), (ii) the isolated  kinase domain in the absence of the  SH3 and SH2 domains bound to PP1  (green), and (iii) the isolated kinase domain in the  absence of PP1 (red).	bind
54265	4	4366	6	NULL	NULL	NULL	NULL	statement 3			in the absence of								SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_105_1_115_s_84	11301007	(Bottom) Fluctuations  in the simulation of three states of  the enzyme: (i) The inactive and assembled structure (including  SH2 and SH3) bound to PP1 (blue), (ii) the isolated  kinase domain in the absence of the  SH3 and SH2 domains bound to PP1  (green), and (iii) the isolated kinase domain in the  absence of PP1 (red).	bind
54266	5	4366	6	10	NULL	0	NULL	statement 3			in the absence of								SH2 domain		NULL		0	NULL	NULL	NULL	gw60_cell_105_1_115_s_84	11301007	(Bottom) Fluctuations  in the simulation of three states of  the enzyme: (i) The inactive and assembled structure (including  SH2 and SH3) bound to PP1 (blue), (ii) the isolated  kinase domain in the absence of the  SH3 and SH2 domains bound to PP1  (green), and (iii) the isolated kinase domain in the  absence of PP1 (red).	bind
10881	1	4367	5	10	NULL	0	NULL	Bmp Smads	NULL		bind	NULL	specifically				NULL			SBE	NULL	embryonic hindlimb 	NULL	NULL	NULL	NULL	gw70_development_133_8_1575_s_239	16556916	(Bottom) In vivo ChIP analysis utilizing extracts from  embryonic hindlimb and an antibody specific for Bmp Smads demonstrated specific binding  of Bmp Smads to a region containing the Smad binding element (SBE; 2).	bind
10882	2	4367	5	NULL	NULL	0	NULL	SBE	NULL		is	NULL				Smad binding element	NULL				NULL		0	NULL	NULL	NULL	gw70_development_133_8_1575_s_239	16556916	(Bottom) In vivo ChIP analysis utilizing extracts from  embryonic hindlimb and an antibody specific for Bmp Smads demonstrated specific binding  of Bmp Smads to a region containing the Smad binding element (SBE; 2).	bind
9969	1	4367	6	NULL	NULL	NULL	NULL	Bmp Smads	GP		bind		specifically							SBE	NULL	extracts from embryonic hindlimb	NULL	NULL	NULL	NULL	gw70_development_133_8_1575_s_239	16556916	(Bottom) In vivo ChIP analysis utilizing extracts from  embryonic hindlimb and an antibody specific for Bmp Smads demonstrated specific binding  of Bmp Smads to a region containing the Smad binding element (SBE; 2).	bind
9970	2	4367	6	NULL	NULL	0	NULL	SBE	NULL		is	NULL				Smad binding element	NULL				NULL		0	NULL	NULL	NULL	gw70_development_133_8_1575_s_239	16556916	(Bottom) In vivo ChIP analysis utilizing extracts from  embryonic hindlimb and an antibody specific for Bmp Smads demonstrated specific binding  of Bmp Smads to a region containing the Smad binding element (SBE; 2).	bind
10883	1	4368	5	NULL	NULL	0	NULL	RNA	NULL		bind	NULL					NULL		RBD (E29C) 		NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_9_1899_s_171	10756189	(Bottom) Representative plot of fraction RNA bound by RBD (E29C) as a function of protein concentration.	bind
9971	1	4368	6	NULL	NULL	NULL	NULL	 RNA	NucleicAcid		bind								RBD (E29C)		NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_9_1899_s_171	10756189	(Bottom) Representative plot of fraction RNA bound by RBD (E29C) as a function of protein concentration.	bind
10887	1	4371	5	NULL	NULL	0	NULL	K+ channel Kv1.4	NULL		bind	NULL	specifically			PSD-95	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_24_3_659_s_46	10595517	(Bottom) Western blotting shows that the K+ channel Kv1.4 also specifically binds to the PSD-95 column.	bind
9972	1	4371	6	NULL	NULL	NULL	NULL	K+ channel Kv1.4	GP		bind		specifically			PSD-95	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_24_3_659_s_46	10595517	(Bottom) Western blotting shows that the K+ channel Kv1.4 also specifically binds to the PSD-95 column.	bind
10889	1	4373	5	10	NULL	0	NULL	L. monocytogenes genome			contain					target sites for CcpC regulation				between positions - 300 and +100 to translational start site	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_1_179_s_162	16352834	(Box I: ATAA-N7-TTAT) ( ). Using this CcpC consensus binding site, we searched the  L. monocytogenes genome and identified 92 potential target sites for CcpC regulation located between positions  - 300 and +100 with respect to a translational start site.	bind
12781	1	4373	6	NULL	NULL	NULL	NULL	L. monocytogenes genome	Organism		contains					targets sites for CcpC regulation	GP			between positions - 300 and +100 to translational start site	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_1_179_s_162	16352834	(Box I: ATAA-N7-TTAT) ( ). Using this CcpC consensus binding site, we searched the  L. monocytogenes genome and identified 92 potential target sites for CcpC regulation located between positions  - 300 and +100 with respect to a translational start site.	bind
10892	1	4376	5	NULL	NULL	0	NULL	tropomyosin	NULL		bind	NULL				actin-myosin S-1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_22_12867_s_68	8662810	(By equilibrium linkage ( 6,  7) this in turn implies that troponin promotes tropomyosin binding to actin-myosin S-1.)	bind
10893	2	4376	5	NULL	NULL	0	NULL	troponin	NULL		promote	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_22_12867_s_68	8662810	(By equilibrium linkage ( 6,  7) this in turn implies that troponin promotes tropomyosin binding to actin-myosin S-1.)	bind
9973	1	4376	6	NULL	NULL	NULL	NULL	tropomyosin	GP		bind					actin-myosin S-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_12867_s_68	8662810	(By equilibrium linkage ( 6,  7) this in turn implies that troponin promotes tropomyosin binding to actin-myosin S-1.)	bind
9974	2	4376	6	NULL	NULL	NULL	NULL	troponin	GP		promotes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_12867_s_68	8662810	(By equilibrium linkage ( 6,  7) this in turn implies that troponin promotes tropomyosin binding to actin-myosin S-1.)	bind
10896	1	4377	5	NULL	NULL	0	NULL	E. coli	NULL		bind	NULL				BECs	NULL	human			NULL		0	NULL	NULL	NULL	gw70_infectimmun_73_4_1947_s_142	15784534	(C  and D) Binding of  E. coli to human BECs visualized by using rhodamine-labeled  A. actinomycetemcomitans against a fluorescein-cytokeratin-labeled BEC background.	bind
9975	1	4377	6	NULL	NULL	NULL	NULL	E.coli	Organism		bind					BECs	Cell	human			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_4_1947_s_142	15784534	(C  and D) Binding of  E. coli to human BECs visualized by using rhodamine-labeled  A. actinomycetemcomitans against a fluorescein-cytokeratin-labeled BEC background.	bind
10897	1	4378	5	NULL	NULL	0	NULL	COS cells	NULL		express	NULL				neuropilin	NULL	rat			NULL		0	NULL	NULL	NULL	gw60_cell_90_4_739_s_90	9288753	(C - H) Binding of various AP  fusion proteins to COS cells expressing rat neuropilin.	bind
10898	2	4378	5	NULL	NULL	0	NULL	AP fusion proteins	NULL		bind	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_90_4_739_s_90	9288753	(C - H) Binding of various AP  fusion proteins to COS cells expressing rat neuropilin.	bind
9995	2	4378	6	NULL	NULL	NULL	NULL	AP fusion proteins	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_90_4_739_s_90	9288753	(C - H) Binding of various AP  fusion proteins to COS cells expressing rat neuropilin.	bind
54267	1	4378	6	NULL	NULL	NULL	NULL	COS cells	Cell		express					neuropilin	GP	rat			NULL		NULL	NULL	NULL	NULL	gw60_cell_90_4_739_s_90	9288753	(C - H) Binding of various AP  fusion proteins to COS cells expressing rat neuropilin.	bind
10899	1	4379	5	10	NULL	0	NULL	Tbx5	NULL		bind	NULL				 ANF	NULL			TBE	NULL		NULL	NULL	NULL	NULL	gw60_cell_106_6_709_s_188	11572777	(C and  D) Tbx5 binds to the  ANF and  cx40  TBEs.	bind
10901	2	4379	5	10	NULL	0	NULL	Tbx5	NULL		bind	NULL				cx40	NULL			TBE	NULL		NULL	NULL	NULL	NULL	gw60_cell_106_6_709_s_188	11572777	(C and  D) Tbx5 binds to the  ANF and  cx40  TBEs.	bind
9996	1	4379	6	NULL	NULL	NULL	NULL	Tbx5	GP		bind					ANF	GP			TBE	NULL		NULL	NULL	NULL	NULL	gw60_cell_106_6_709_s_188	11572777	(C and  D) Tbx5 binds to the  ANF and  cx40  TBEs.	bind
9997	2	4379	6	NULL	NULL	NULL	NULL	Tbx5	GP		bind					cx40	GP			TBE	NULL		NULL	NULL	NULL	NULL	gw60_cell_106_6_709_s_188	11572777	(C and  D) Tbx5 binds to the  ANF and  cx40  TBEs.	bind
10902	1	4380	5	NULL	NULL	0	NULL	Raf-1	NULL		bind	NULL				Rb	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_177	15485920	(C and D)  The presence of 1 muM penetratin-Raf-1 peptide conjugate markedly inhibits the binding  of Raf-1 to Rb (C), whereas a scrambled peptide conjugate is unable to do so (D).	bind
10903	2	4380	5	NULL	NULL	0	NULL	penetratin-Raf-1 peptide conjugate	NULL		inhibit	NULL	markedly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_177	15485920	(C and D)  The presence of 1 muM penetratin-Raf-1 peptide conjugate markedly inhibits the binding  of Raf-1 to Rb (C), whereas a scrambled peptide conjugate is unable to do so (D).	bind
10904	3	4380	5	NULL	NULL	0	NULL	scrambled peptide conjugate	NULL		does not inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_177	15485920	(C and D)  The presence of 1 muM penetratin-Raf-1 peptide conjugate markedly inhibits the binding  of Raf-1 to Rb (C), whereas a scrambled peptide conjugate is unable to do so (D).	bind
9998	1	4380	6	NULL	NULL	NULL	NULL	Raf-1	GP		bind					Rb	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_177	15485920	(C and D)  The presence of 1 muM penetratin-Raf-1 peptide conjugate markedly inhibits the binding  of Raf-1 to Rb (C), whereas a scrambled peptide conjugate is unable to do so (D).	bind
9999	2	4380	6	NULL	NULL	NULL	NULL	penetratin-Raf-1 peptide 	AminoAcid		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_177	15485920	(C and D)  The presence of 1 muM penetratin-Raf-1 peptide conjugate markedly inhibits the binding  of Raf-1 to Rb (C), whereas a scrambled peptide conjugate is unable to do so (D).	bind
10000	3	4380	6	NULL	NULL	NULL	NULL	scrambled peptide conjugate	AminoAcid		does not inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_177	15485920	(C and D)  The presence of 1 muM penetratin-Raf-1 peptide conjugate markedly inhibits the binding  of Raf-1 to Rb (C), whereas a scrambled peptide conjugate is unable to do so (D).	bind
10905	1	4381	5	NULL	NULL	0	NULL	AfaF	NULL		bind	NULL				Lrp	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_185_6_1886_s_229	12618452	(C and D) AfaF bound to Lrp allows Lrp binding to GATCdist in phase-ON cells (C) and increases Lrp binding to GATCprox in phase-OFF cells (D).	bind
10909	2	4381	5	NULL	NULL	0	NULL	Lrp	NULL		bind	NULL					NULL			GATCdist	NULL	phase-ON cells	0	NULL	NULL	NULL	gw60_jbacteriol_185_6_1886_s_229	12618452	(C and D) AfaF bound to Lrp allows Lrp binding to GATCdist in phase-ON cells (C) and increases Lrp binding to GATCprox in phase-OFF cells (D).	bind
10911	3	4381	5	NULL	NULL	0	NULL	statement 1	NULL		allows	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_185_6_1886_s_229	12618452	(C and D) AfaF bound to Lrp allows Lrp binding to GATCdist in phase-ON cells (C) and increases Lrp binding to GATCprox in phase-OFF cells (D).	bind
10913	4	4381	5	NULL	NULL	0	NULL	Lrp	NULL		bind	NULL					NULL			GATCprox	NULL	phase-OFF cells	0	NULL	NULL	NULL	gw60_jbacteriol_185_6_1886_s_229	12618452	(C and D) AfaF bound to Lrp allows Lrp binding to GATCdist in phase-ON cells (C) and increases Lrp binding to GATCprox in phase-OFF cells (D).	bind
10914	5	4381	5	NULL	NULL	0	NULL	statement 1	NULL		increase	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_185_6_1886_s_229	12618452	(C and D) AfaF bound to Lrp allows Lrp binding to GATCdist in phase-ON cells (C) and increases Lrp binding to GATCprox in phase-OFF cells (D).	bind
10001	1	4381	6	NULL	NULL	NULL	NULL	AfaF	GP		bind					Lrp	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_6_1886_s_229	12618452	(C and D) AfaF bound to Lrp allows Lrp binding to GATCdist in phase-ON cells (C) and increases Lrp binding to GATCprox in phase-OFF cells (D).	bind
10002	2	4381	6	NULL	NULL	NULL	NULL	Lrp	GP		bind									GATCdist	NULL	phase-ON cells	NULL	NULL	NULL	NULL	gw60_jbacteriol_185_6_1886_s_229	12618452	(C and D) AfaF bound to Lrp allows Lrp binding to GATCdist in phase-ON cells (C) and increases Lrp binding to GATCprox in phase-OFF cells (D).	bind
10003	3	4381	6	NULL	NULL	NULL	NULL	Lrp	GP		bind									GATCprox	NULL	phase-OFF cells	NULL	NULL	NULL	NULL	gw60_jbacteriol_185_6_1886_s_229	12618452	(C and D) AfaF bound to Lrp allows Lrp binding to GATCdist in phase-ON cells (C) and increases Lrp binding to GATCprox in phase-OFF cells (D).	bind
10004	4	4381	6	NULL	NULL	NULL	NULL	statement 1	Process		allows					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_6_1886_s_229	12618452	(C and D) AfaF bound to Lrp allows Lrp binding to GATCdist in phase-ON cells (C) and increases Lrp binding to GATCprox in phase-OFF cells (D).	bind
10005	5	4381	6	NULL	NULL	NULL	NULL	statement 1	Process		increases					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_6_1886_s_229	12618452	(C and D) AfaF bound to Lrp allows Lrp binding to GATCdist in phase-ON cells (C) and increases Lrp binding to GATCprox in phase-OFF cells (D).	bind
10941	1	4382	5	NULL	NULL	0	NULL	E(spl)bHLH proteins	NULL		bind	NULL				B1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_7_4600_s_149	10373509	(C and D) Binding of E(spl)bHLH proteins to B1, A1, and A2 (Table  1).	bind
10942	2	4382	5	NULL	NULL	0	NULL	E(spl)bHLH proteins	NULL		bind	NULL				A1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_7_4600_s_149	10373509	(C and D) Binding of E(spl)bHLH proteins to B1, A1, and A2 (Table  1).	bind
10943	3	4382	5	NULL	NULL	0	NULL	E(spl)bHLH proteins	NULL		bind	NULL				A2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_7_4600_s_149	10373509	(C and D) Binding of E(spl)bHLH proteins to B1, A1, and A2 (Table  1).	bind
10795	1	4382	6	NULL	NULL	NULL	NULL	E(spl)bHLH proteins	GP		bind					B1					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4600_s_149	10373509	(C and D) Binding of E(spl)bHLH proteins to B1, A1, and A2 (Table  1).	bind
10796	2	4382	6	NULL	NULL	NULL	NULL	E(spl)bHLH proteins	GP		bind					A1					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4600_s_149	10373509	(C and D) Binding of E(spl)bHLH proteins to B1, A1, and A2 (Table  1).	bind
10797	3	4382	6	NULL	NULL	NULL	NULL	E(spl)bHLH proteins	GP		bind					A2					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4600_s_149	10373509	(C and D) Binding of E(spl)bHLH proteins to B1, A1, and A2 (Table  1).	bind
10944	1	4383	5	NULL	NULL	0	NULL	Bl	NULL		bind	NULL				ribonucleotide homopolymers	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_11_7846_s_145	10523673	(C and D) Binding of the Bl and human K proteins to ribonucleotide homopolymers.	bind
10945	2	4383	5	NULL	NULL	0	NULL	K proteins	NULL	human	bind	NULL				ribonucleotide homopolymers	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_11_7846_s_145	10523673	(C and D) Binding of the Bl and human K proteins to ribonucleotide homopolymers.	bind
10127	1	4383	6	NULL	NULL	NULL	NULL	B1			bind					ribonucleotide polymers	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_11_7846_s_145	10523673	(C and D) Binding of the Bl and human K proteins to ribonucleotide homopolymers.	bind
10128	2	4383	6	NULL	NULL	NULL	NULL	K protein	GP	human	bind					ribonucleotide polymers	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_11_7846_s_145	10523673	(C and D) Binding of the Bl and human K proteins to ribonucleotide homopolymers.	bind
11602	1	4384	5	NULL	NULL	0	NULL	myc-Gcn4p	NULL		bind	NULL				ARG1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8829_s_79	14612422	(C and D) ChIP analysis was conducted as described above to measure binding  of myc-Gcn4p to  ARG1 (C) or  SNZ1 (D) in the following strains: transformants of the  gcn4delta strains containing either all WT SWI/SNF genes (249),  snf2delta (SY169),  swi3delta (SY294),  snf6delta (SY295),  snf11delta (SY296),  snf5delta (SY327), or  swp73delta (SY298), all bearing single-copy plasmid pSK1 containing  GCN4-myc, lanes 2 through 8;  gcn4delta strain (249) transformed with empty vector YCp50 or single-copy plasmid pSY284 containing   gcn4-14Ala-myc, respectively, lanes 1 and 9.	bind
11603	2	4384	5	NULL	NULL	0	NULL	myc-Gcn4p	NULL		bind	NULL				SNZ1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8829_s_79	14612422	(C and D) ChIP analysis was conducted as described above to measure binding  of myc-Gcn4p to  ARG1 (C) or  SNZ1 (D) in the following strains: transformants of the  gcn4delta strains containing either all WT SWI/SNF genes (249),  snf2delta (SY169),  swi3delta (SY294),  snf6delta (SY295),  snf11delta (SY296),  snf5delta (SY327), or  swp73delta (SY298), all bearing single-copy plasmid pSK1 containing  GCN4-myc, lanes 2 through 8;  gcn4delta strain (249) transformed with empty vector YCp50 or single-copy plasmid pSY284 containing   gcn4-14Ala-myc, respectively, lanes 1 and 9.	bind
11604	3	4384	5	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8829_s_79	14612422	(C and D) ChIP analysis was conducted as described above to measure binding  of myc-Gcn4p to  ARG1 (C) or  SNZ1 (D) in the following strains: transformants of the  gcn4delta strains containing either all WT SWI/SNF genes (249),  snf2delta (SY169),  swi3delta (SY294),  snf6delta (SY295),  snf11delta (SY296),  snf5delta (SY327), or  swp73delta (SY298), all bearing single-copy plasmid pSK1 containing  GCN4-myc, lanes 2 through 8;  gcn4delta strain (249) transformed with empty vector YCp50 or single-copy plasmid pSY284 containing   gcn4-14Ala-myc, respectively, lanes 1 and 9.	bind
10798	1	4384	6	NULL	NULL	NULL	NULL	myc-Gcn4p	GP		bind					ARG1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8829_s_79	14612422	(C and D) ChIP analysis was conducted as described above to measure binding  of myc-Gcn4p to  ARG1 (C) or  SNZ1 (D) in the following strains: transformants of the  gcn4delta strains containing either all WT SWI/SNF genes (249),  snf2delta (SY169),  swi3delta (SY294),  snf6delta (SY295),  snf11delta (SY296),  snf5delta (SY327), or  swp73delta (SY298), all bearing single-copy plasmid pSK1 containing  GCN4-myc, lanes 2 through 8;  gcn4delta strain (249) transformed with empty vector YCp50 or single-copy plasmid pSY284 containing   gcn4-14Ala-myc, respectively, lanes 1 and 9.	bind
10799	2	4384	6	NULL	NULL	NULL	NULL	myc-Gcn4p	GP		bind					SNZ1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8829_s_79	14612422	(C and D) ChIP analysis was conducted as described above to measure binding  of myc-Gcn4p to  ARG1 (C) or  SNZ1 (D) in the following strains: transformants of the  gcn4delta strains containing either all WT SWI/SNF genes (249),  snf2delta (SY169),  swi3delta (SY294),  snf6delta (SY295),  snf11delta (SY296),  snf5delta (SY327), or  swp73delta (SY298), all bearing single-copy plasmid pSK1 containing  GCN4-myc, lanes 2 through 8;  gcn4delta strain (249) transformed with empty vector YCp50 or single-copy plasmid pSY284 containing   gcn4-14Ala-myc, respectively, lanes 1 and 9.	bind
10800	3	4384	6	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8829_s_79	14612422	(C and D) ChIP analysis was conducted as described above to measure binding  of myc-Gcn4p to  ARG1 (C) or  SNZ1 (D) in the following strains: transformants of the  gcn4delta strains containing either all WT SWI/SNF genes (249),  snf2delta (SY169),  swi3delta (SY294),  snf6delta (SY295),  snf11delta (SY296),  snf5delta (SY327), or  swp73delta (SY298), all bearing single-copy plasmid pSK1 containing  GCN4-myc, lanes 2 through 8;  gcn4delta strain (249) transformed with empty vector YCp50 or single-copy plasmid pSY284 containing   gcn4-14Ala-myc, respectively, lanes 1 and 9.	bind
10946	1	4385	5	NULL	NULL	0	NULL	T1 reovirus strains	NULL		bind	NULL				NT2 cells	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_104_3_441_s_110	11239401	(C and D) Effect of anti-hJAM mAbs on binding of T1 and T3 reovirus strains to NT2 cells.	bind
10947	2	4385	5	NULL	NULL	0	NULL	T3 reovirus strains	NULL		bind	NULL				NT2 cells	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_104_3_441_s_110	11239401	(C and D) Effect of anti-hJAM mAbs on binding of T1 and T3 reovirus strains to NT2 cells.	bind
10130	1	4385	6	NULL	NULL	NULL	NULL	T1 reovirus	Organism		bind					NT2 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_cell_104_3_441_s_110	11239401	(C and D) Effect of anti-hJAM mAbs on binding of T1 and T3 reovirus strains to NT2 cells.	bind
10131	2	4385	6	NULL	NULL	NULL	NULL	T3 reovirus	Organism		bind					NT2 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_cell_104_3_441_s_110	11239401	(C and D) Effect of anti-hJAM mAbs on binding of T1 and T3 reovirus strains to NT2 cells.	bind
10950	1	4386	5	NULL	NULL	0	NULL	P300 protein	NULL	endogenous	bind	NULL				p53 protein isoforms	NULL	total			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_298	14612423	(C and D) Endogenous P300 protein was immunoprecipitated with an anti-p300  antibody, and levels of total p53 protein isoforms (C) or acetylated p53 isoforms  (D) bound to p300 were quantitated by immunoblotting with either the acetylation-specific  antibody or a p53 protein antibody to normalize to the total p53 protein.	bind
10951	2	4386	5	NULL	NULL	0	NULL	P300 protein	NULL	endogenous	bind	NULL				p53 protein isoforms	NULL	acetylated			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_298	14612423	(C and D) Endogenous P300 protein was immunoprecipitated with an anti-p300  antibody, and levels of total p53 protein isoforms (C) or acetylated p53 isoforms  (D) bound to p300 were quantitated by immunoblotting with either the acetylation-specific  antibody or a p53 protein antibody to normalize to the total p53 protein.	bind
10132	1	4386	6	NULL	NULL	NULL	NULL	p53	GP	acetylated	bind					p300	GP	endogenous			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_298	14612423	(C and D) Endogenous P300 protein was immunoprecipitated with an anti-p300  antibody, and levels of total p53 protein isoforms (C) or acetylated p53 isoforms  (D) bound to p300 were quantitated by immunoblotting with either the acetylation-specific  antibody or a p53 protein antibody to normalize to the total p53 protein.	bind
12782	2	4386	6	NULL	NULL	NULL	NULL	p53	GP	total	bind					p300	GP	endogenous			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_298	14612423	(C and D) Endogenous P300 protein was immunoprecipitated with an anti-p300  antibody, and levels of total p53 protein isoforms (C) or acetylated p53 isoforms  (D) bound to p300 were quantitated by immunoblotting with either the acetylation-specific  antibody or a p53 protein antibody to normalize to the total p53 protein.	bind
10952	1	4387	5	10	NULL	0	NULL	Etheno-ATP			bind					Arp2/3 complex		purified;;mutant			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_2_315_s_81	15657399	(C and D) Etheno-ATP binding to purified Arp2/3 complex mutants.	bind
10134	1	4387	6	NULL	NULL	NULL	NULL	Etheno-ATP	Chemical		bind					Arp2/3 complex	GP	purified;;mutant			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_2_315_s_81	15657399	(C and D) Etheno-ATP binding to purified Arp2/3 complex mutants.	bind
10953	1	4388	5	NULL	NULL	0	NULL	GADD34	NULL		bind	NULL				Smad7	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_164_2_291_s_76	14718519	(c and d) Experiments were performed in both yeast  (c) and mammalian (d) systems, as in  Fig. 1, to map GADD34 binding to Smad7.	bind
10135	1	4388	6	NULL	NULL	NULL	NULL	GADD34	GP		bind					Smad7	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_291_s_76	14718519	(c and d) Experiments were performed in both yeast  (c) and mammalian (d) systems, as in  Fig. 1, to map GADD34 binding to Smad7.	bind
10954	1	4389	5	10	NULL	0	NULL	plasmid p28			confers					Sema III		binding activity of			NULL		NULL	NULL	NULL	NULL	gw60_cell_90_4_739_s_67	9288753	(C and D) Following isolation of plasmid p28, which confers Sema III - binding  activity, Sema III - AP (D) but not AP (C) was found to bind cells transiently transfected  with p28.	bind
10955	3	4389	5	NULL	NULL	0	NULL	Sema III - AP	NULL		bind	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cell_90_4_739_s_67	9288753	(C and D) Following isolation of plasmid p28, which confers Sema III - binding  activity, Sema III - AP (D) but not AP (C) was found to bind cells transiently transfected  with p28.	bind
10956	4	4389	5	NULL	NULL	0	NULL	AP	NULL		does not bind	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cell_90_4_739_s_67	9288753	(C and D) Following isolation of plasmid p28, which confers Sema III - binding  activity, Sema III - AP (D) but not AP (C) was found to bind cells transiently transfected  with p28.	bind
44439	2	4389	5	10	NULL	0	NULL	cells	NULL		transfected with	NULL	transiently			p28	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_90_4_739_s_67	9288753	(C and D) Following isolation of plasmid p28, which confers Sema III - binding  activity, Sema III - AP (D) but not AP (C) was found to bind cells transiently transfected  with p28.	bind
10801	1	4389	6	NULL	NULL	NULL	NULL	p28	GP		confers					SemaIII	GP	binding activity of			NULL		NULL	NULL	NULL	NULL	gw60_cell_90_4_739_s_67	9288753	(C and D) Following isolation of plasmid p28, which confers Sema III - binding  activity, Sema III - AP (D) but not AP (C) was found to bind cells transiently transfected  with p28.	bind
10802	2	4389	6	NULL	NULL	NULL	NULL	cells	Cell		transfected with		transiently			p28	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_90_4_739_s_67	9288753	(C and D) Following isolation of plasmid p28, which confers Sema III - binding  activity, Sema III - AP (D) but not AP (C) was found to bind cells transiently transfected  with p28.	bind
11663	3	4389	6	NULL	NULL	NULL	NULL	Sema III - AP	GP		bind					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_90_4_739_s_67	9288753	(C and D) Following isolation of plasmid p28, which confers Sema III - binding  activity, Sema III - AP (D) but not AP (C) was found to bind cells transiently transfected  with p28.	bind
54285	4	4389	6	NULL	NULL	NULL	NULL	AP	GP		does not bind					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_90_4_739_s_67	9288753	(C and D) Following isolation of plasmid p28, which confers Sema III - binding  activity, Sema III - AP (D) but not AP (C) was found to bind cells transiently transfected  with p28.	bind
10957	1	4390	5	NULL	NULL	0	NULL	EhRab7A	NULL	recombinant	bind	NULL				EhVps26	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molbiolcell_16_11_5294_s_149	16120649	(C and D) In vitro binding of recombinant EhRab7A with EhVps26  and EhVps29 (C), and of recombinant EhRab7A with EhVps26FL and EhVps26deltaC (D).	bind
10958	2	4390	5	NULL	NULL	0	NULL	EhRab7A	NULL	recombinant	bind	NULL				EhVps29	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molbiolcell_16_11_5294_s_149	16120649	(C and D) In vitro binding of recombinant EhRab7A with EhVps26  and EhVps29 (C), and of recombinant EhRab7A with EhVps26FL and EhVps26deltaC (D).	bind
10959	3	4390	5	10	NULL	0	NULL	EhRab7A		recombinant	bind					EhVps26FL					NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molbiolcell_16_11_5294_s_149	16120649	(C and D) In vitro binding of recombinant EhRab7A with EhVps26  and EhVps29 (C), and of recombinant EhRab7A with EhVps26FL and EhVps26deltaC (D).	bind
10960	4	4390	5	10	NULL	0	NULL	EhRab7A		recombinant	bind					EhVps26deltaC					NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molbiolcell_16_11_5294_s_149	16120649	(C and D) In vitro binding of recombinant EhRab7A with EhVps26  and EhVps29 (C), and of recombinant EhRab7A with EhVps26FL and EhVps26deltaC (D).	bind
10137	1	4390	6	NULL	NULL	NULL	NULL	EhRab7A	GP	recombinant	bind					EhVps26	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molbiolcell_16_11_5294_s_149	16120649	(C and D) In vitro binding of recombinant EhRab7A with EhVps26  and EhVps29 (C), and of recombinant EhRab7A with EhVps26FL and EhVps26deltaC (D).	bind
10138	2	4390	6	NULL	NULL	NULL	NULL	EhVps7A	GP	recombinant	bind					Ehvps29	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molbiolcell_16_11_5294_s_149	16120649	(C and D) In vitro binding of recombinant EhRab7A with EhVps26  and EhVps29 (C), and of recombinant EhRab7A with EhVps26FL and EhVps26deltaC (D).	bind
10139	3	4390	6	NULL	NULL	NULL	NULL	EhRab7A	GP	recombinant	bind					EhVps26FL	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molbiolcell_16_11_5294_s_149	16120649	(C and D) In vitro binding of recombinant EhRab7A with EhVps26  and EhVps29 (C), and of recombinant EhRab7A with EhVps26FL and EhVps26deltaC (D).	bind
10140	4	4390	6	NULL	NULL	NULL	NULL	EhRab7A	GP	recombinant	bind					EhVps26deltaC 	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molbiolcell_16_11_5294_s_149	16120649	(C and D) In vitro binding of recombinant EhRab7A with EhVps26  and EhVps29 (C), and of recombinant EhRab7A with EhVps26FL and EhVps26deltaC (D).	bind
10961	1	4391	5	NULL	NULL	0	NULL	SsrA peptide	NULL		bind	NULL				SspB	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_12_1_75_s_50	12887894	(C and D) Isothermal titration calorimetric studies of SsrA peptide binding to SspB (C) and SspB127 (D) reveal dissociation constants of 6.16 and 6.22  M, respectively.	bind
10962	2	4391	5	NULL	NULL	0	NULL	SsrA peptide	NULL		bind	NULL				SspB127	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_12_1_75_s_50	12887894	(C and D) Isothermal titration calorimetric studies of SsrA peptide binding to SspB (C) and SspB127 (D) reveal dissociation constants of 6.16 and 6.22  M, respectively.	bind
10145	1	4391	6	NULL	NULL	NULL	NULL	SsrA peptide	GP		bind					SspB	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_75_s_50	12887894	(C and D) Isothermal titration calorimetric studies of SsrA peptide binding to SspB (C) and SspB127 (D) reveal dissociation constants of 6.16 and 6.22  M, respectively.	bind
10146	2	4391	6	NULL	NULL	NULL	NULL	SsrA peptide	GP		bind					SspB127	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_75_s_50	12887894	(C and D) Isothermal titration calorimetric studies of SsrA peptide binding to SspB (C) and SspB127 (D) reveal dissociation constants of 6.16 and 6.22  M, respectively.	bind
10963	1	4392	5	NULL	NULL	0	NULL	type IV collagen	NULL		bind	NULL				fibronectin	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_10_4467_s_137	15282337	(C and D) Quantification of type IV collagen binding to fibronectin beads (including  means and standard deviations of four experiments).	bind
10147	1	4392	6	NULL	NULL	NULL	NULL	type IV collagen	GP		bind					fibronectin beads	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_10_4467_s_137	15282337	(C and D) Quantification of type IV collagen binding to fibronectin beads (including  means and standard deviations of four experiments).	bind
10964	1	4393	5	NULL	NULL	0	NULL	Rad24p	NULL		bind	NULL				Eco1p	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_8_2999_s_162	12665596	(C and D) Rad24p binding to Eco1p was  not disrupted by DNase I treatment, while this level of DNase I under identical conditions  was sufficient to completely digest 500 ng of lambda DNA.	bind
10965	2	4393	5	10	NULL	0	NULL	DNase I			does not disrupt					statement 1					NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2999_s_162	12665596	(C and D) Rad24p binding to Eco1p was  not disrupted by DNase I treatment, while this level of DNase I under identical conditions  was sufficient to completely digest 500 ng of lambda DNA.	bind
10966	3	4393	5	10	NULL	0	NULL	DNase I			digest		completely			lambda DNA					NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2999_s_162	12665596	(C and D) Rad24p binding to Eco1p was  not disrupted by DNase I treatment, while this level of DNase I under identical conditions  was sufficient to completely digest 500 ng of lambda DNA.	bind
10265	1	4393	6	NULL	NULL	NULL	NULL	Rad24p	GP		bind					Eco1p	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2999_s_162	12665596	(C and D) Rad24p binding to Eco1p was  not disrupted by DNase I treatment, while this level of DNase I under identical conditions  was sufficient to completely digest 500 ng of lambda DNA.	bind
10266	2	4393	6	NULL	NULL	NULL	NULL	DNase I	GP		does not disrupt					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2999_s_162	12665596	(C and D) Rad24p binding to Eco1p was  not disrupted by DNase I treatment, while this level of DNase I under identical conditions  was sufficient to completely digest 500 ng of lambda DNA.	bind
54286	3	4393	6	NULL	NULL	NULL	NULL	DNase I 	GP		digest		completely			lambda DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_8_2999_s_162	12665596	(C and D) Rad24p binding to Eco1p was  not disrupted by DNase I treatment, while this level of DNase I under identical conditions  was sufficient to completely digest 500 ng of lambda DNA.	bind
10967	1	4395	5	10	NULL	0	NULL	 fra-1 			bind					fra-1				TRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_12_4401_s_230	12773579	(C and D) Serum induction of  fra-1 and mRNA and protein binding to  fra-1 TRE.	bind
10970	2	4395	5	10	NULL	0	NULL	serum			induce					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_12_4401_s_230	12773579	(C and D) Serum induction of  fra-1 and mRNA and protein binding to  fra-1 TRE.	bind
10269	1	4395	6	NULL	NULL	NULL	NULL	Fra-1	GP		bind					fra-1	GP			TRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_12_4401_s_230	12773579	(C and D) Serum induction of  fra-1 and mRNA and protein binding to  fra-1 TRE.	bind
10273	2	4395	6	NULL	NULL	NULL	NULL	serum	Chemical		induces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_12_4401_s_230	12773579	(C and D) Serum induction of  fra-1 and mRNA and protein binding to  fra-1 TRE.	bind
10971	1	4396	5	NULL	NULL	0	NULL	Ste12	NULL		bind	NULL				filamentation genes	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_113_3_395_s_133	12732146	(C and D) Ste12 binding to filamentation genes during butanol treatment.	bind
10972	2	4396	5	10	NULL	0	NULL	statement 1			occurs during					butanol		treatment with			NULL		NULL	NULL	NULL	NULL	gw60_cell_113_3_395_s_133	12732146	(C and D) Ste12 binding to filamentation genes during butanol treatment.	bind
10276	1	4396	6	NULL	NULL	NULL	NULL	Ste12	GP		bind					filamentous genes	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_113_3_395_s_133	12732146	(C and D) Ste12 binding to filamentation genes during butanol treatment.	bind
10277	2	4396	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs during					butanol	Chemical	treatment with			NULL		NULL	NULL	NULL	NULL	gw60_cell_113_3_395_s_133	12732146	(C and D) Ste12 binding to filamentation genes during butanol treatment.	bind
10973	1	4397	5	10	NULL	0	NULL	 DR		nuclear	bind					hsp90					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5811_s_174	10409767	(c and d) The nuclear DR remains bound to hsp90.	bind
10278	1	4397	6	NULL	NULL	NULL	NULL	DR	GP	nuclear	bind					hsp90	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5811_s_174	10409767	(c and d) The nuclear DR remains bound to hsp90.	bind
10986	1	4399	5	NULL	NULL	0	NULL	S1-S2-GluR2	NULL		bind	NULL				NR2A	NULL		glutamate		NULL		0	NULL	NULL	NULL	gw60_neuron_32_6_1085_s_264	11754839	(C and D) Three-dimensional model of the ligand binding domain of NR2A (C) and NR1 (D) based on the structure of S1-S2-GluR2 bound to glutamate for NR2A and the apo structure for NR1 (Protein Data Bank ID codes: 1FTJ for NR2A and 1FTO for NR1).	bind
12783	1	4399	6	NULL	NULL	NULL	NULL	S1-S2-GluR2	AminoAcid		bind					NR2A	GP		glutamate		NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_6_1085_s_264	11754839	(C and D) Three-dimensional model of the ligand binding domain of NR2A (C) and NR1 (D) based on the structure of S1-S2-GluR2 bound to glutamate for NR2A and the apo structure for NR1 (Protein Data Bank ID codes: 1FTJ for NR2A and 1FTO for NR1).	bind
10991	1	4400	5	NULL	NULL	0	NULL	myc-Srb6p	NULL		bind	NULL				SNZ1	NULL			UAS	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_15_6871_s_178	15254252	(C and F) The procedures described for panels B and E were employed to analyze  binding of myc-Srb6p (C) or myc-Gal11p (F) to the  SNZ1 UAS.	bind
10994	2	4400	5	NULL	NULL	0	NULL	myc-Gal11p	NULL		bind	NULL				SNZ1	NULL			UAS	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_15_6871_s_178	15254252	(C and F) The procedures described for panels B and E were employed to analyze  binding of myc-Srb6p (C) or myc-Gal11p (F) to the  SNZ1 UAS.	bind
13105	3	4400	5	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_15_6871_s_178	15254252	(C and F) The procedures described for panels B and E were employed to analyze  binding of myc-Srb6p (C) or myc-Gal11p (F) to the  SNZ1 UAS.	bind
10282	1	4400	6	NULL	NULL	NULL	NULL	myc-Srb6p	GP		bind					SNZ1	GP			UAS	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_15_6871_s_178	15254252	(C and F) The procedures described for panels B and E were employed to analyze  binding of myc-Srb6p (C) or myc-Gal11p (F) to the  SNZ1 UAS.	bind
10283	2	4400	6	NULL	NULL	NULL	NULL	myc-Gal11p	GP		bind					SNZ1	GP			UAS	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_15_6871_s_178	15254252	(C and F) The procedures described for panels B and E were employed to analyze  binding of myc-Srb6p (C) or myc-Gal11p (F) to the  SNZ1 UAS.	bind
10284	3	4400	6	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_15_6871_s_178	15254252	(C and F) The procedures described for panels B and E were employed to analyze  binding of myc-Srb6p (C) or myc-Gal11p (F) to the  SNZ1 UAS.	bind
10995	1	4401	5	NULL	NULL	0	NULL	phospho-CheY	NULL		bind	NULL				FliM	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_21_5580_s_399	9791106	(C to E) Hypotheses for the movements that might be triggered by binding of phospho-CheY to FliM, to cause switching to the CW direction of motor rotation.	bind
11001	2	4401	5	NULL	NULL	0	NULL	statement 1	NULL		causes	NULL				CW direction of motor rotation	NULL	switching to			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_21_5580_s_399	9791106	(C to E) Hypotheses for the movements that might be triggered by binding of phospho-CheY to FliM, to cause switching to the CW direction of motor rotation.	bind
10285	1	4401	6	NULL	NULL	NULL	NULL	phospho-CheY	GP		bind					FliM	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_21_5580_s_399	9791106	(C to E) Hypotheses for the movements that might be triggered by binding of phospho-CheY to FliM, to cause switching to the CW direction of motor rotation.	bind
12784	2	4401	6	NULL	NULL	NULL	NULL	statement 1	Process		causes					CW direction of motor rotation		switching to			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_21_5580_s_399	9791106	(C to E) Hypotheses for the movements that might be triggered by binding of phospho-CheY to FliM, to cause switching to the CW direction of motor rotation.	bind
11005	1	4402	5	NULL	NULL	0	NULL	Tem1	NULL		bind	NULL				Cdc15	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_112_5_697_s_204	12628189	(C)  AMN1 overexpression inhibits the binding between Tem1 and Cdc15.	bind
11006	2	4402	5	NULL	NULL	0	NULL	AMN1	NULL	overexpression of	inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_112_5_697_s_204	12628189	(C)  AMN1 overexpression inhibits the binding between Tem1 and Cdc15.	bind
10286	1	4402	6	NULL	NULL	NULL	NULL	Tem1	GP		bind					Cdc15	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_5_697_s_204	12628189	(C)  AMN1 overexpression inhibits the binding between Tem1 and Cdc15.	bind
10287	2	4402	6	NULL	NULL	NULL	NULL	AMN1	GP	overexpression of	inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_5_697_s_204	12628189	(C)  AMN1 overexpression inhibits the binding between Tem1 and Cdc15.	bind
11007	1	4403	5	NULL	NULL	0	NULL	nuclear proteins	NULL		bind	NULL				TGF- 1	NULL	human		AP-1 site B of promoter	NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_2_301_s_95	12711314	(C)  Binding of nuclear proteins to the AP-1 site B of the human TGF- 1 promoter.	bind
10288	1	4403	6	NULL	NULL	NULL	NULL	nuclear protein	GP		bind					TGF-1 	GP	human		AP-1 site B of promoter	NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_2_301_s_95	12711314	(C)  Binding of nuclear proteins to the AP-1 site B of the human TGF- 1 promoter.	bind
11008	1	4404	5	NULL	NULL	0	NULL	H3 Ab	NULL		bind	NULL				H3 peptide	NULL	unphosphorylated 			NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_2_225_s_117	10209020	(C)  ELISA of H3 Ab binding to the unphosphorylated H3 peptide  (open square), phosphorylated H3 peptide (closed square), total  cellular proteins from cycling cells (open circle) or from cells  treated with nocodazole (closed circle).	bind
11010	2	4404	5	NULL	NULL	0	NULL	H3 Ab	NULL		bind	NULL				H3 peptide	NULL	phosphorylated			NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_2_225_s_117	10209020	(C)  ELISA of H3 Ab binding to the unphosphorylated H3 peptide  (open square), phosphorylated H3 peptide (closed square), total  cellular proteins from cycling cells (open circle) or from cells  treated with nocodazole (closed circle).	bind
11011	5	4404	5	10	NULL	0	NULL	H3 Ab	NULL		bind	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_2_225_s_117	10209020	(C)  ELISA of H3 Ab binding to the unphosphorylated H3 peptide  (open square), phosphorylated H3 peptide (closed square), total  cellular proteins from cycling cells (open circle) or from cells  treated with nocodazole (closed circle).	bind
11013	6	4404	5	10	NULL	0	NULL	H3 Ab	NULL		bind	NULL				statement 4	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_2_225_s_117	10209020	(C)  ELISA of H3 Ab binding to the unphosphorylated H3 peptide  (open square), phosphorylated H3 peptide (closed square), total  cellular proteins from cycling cells (open circle) or from cells  treated with nocodazole (closed circle).	bind
44440	3	4404	5	10	NULL	0	NULL	total cellular proteins	NULL		are from	NULL				cells treated with nocodazole	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_2_225_s_117	10209020	(C)  ELISA of H3 Ab binding to the unphosphorylated H3 peptide  (open square), phosphorylated H3 peptide (closed square), total  cellular proteins from cycling cells (open circle) or from cells  treated with nocodazole (closed circle).	bind
44441	4	4404	5	10	NULL	0	NULL	total cellular proteins	NULL		are from	NULL				cycling cells	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_2_225_s_117	10209020	(C)  ELISA of H3 Ab binding to the unphosphorylated H3 peptide  (open square), phosphorylated H3 peptide (closed square), total  cellular proteins from cycling cells (open circle) or from cells  treated with nocodazole (closed circle).	bind
10289	1	4404	6	NULL	NULL	NULL	NULL	H3 Ab 	GP		bind					H3 peptide	AminoAcid	unphosphorylated			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_2_225_s_117	10209020	(C)  ELISA of H3 Ab binding to the unphosphorylated H3 peptide  (open square), phosphorylated H3 peptide (closed square), total  cellular proteins from cycling cells (open circle) or from cells  treated with nocodazole (closed circle).	bind
10290	2	4404	6	NULL	NULL	NULL	NULL	H3 Ab	GP		bind					H3 peptide	AminoAcid	phosphorylated			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_2_225_s_117	10209020	(C)  ELISA of H3 Ab binding to the unphosphorylated H3 peptide  (open square), phosphorylated H3 peptide (closed square), total  cellular proteins from cycling cells (open circle) or from cells  treated with nocodazole (closed circle).	bind
10291	3	4404	6	NULL	NULL	NULL	NULL	total cellular proteins	GP		are from					cycling cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_2_225_s_117	10209020	(C)  ELISA of H3 Ab binding to the unphosphorylated H3 peptide  (open square), phosphorylated H3 peptide (closed square), total  cellular proteins from cycling cells (open circle) or from cells  treated with nocodazole (closed circle).	bind
10292	4	4404	6	NULL	NULL	NULL	NULL	total cellular proteins	GP		are from					cells treated with nocodazole	Cell				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_2_225_s_117	10209020	(C)  ELISA of H3 Ab binding to the unphosphorylated H3 peptide  (open square), phosphorylated H3 peptide (closed square), total  cellular proteins from cycling cells (open circle) or from cells  treated with nocodazole (closed circle).	bind
54287	5	4404	6	NULL	NULL	NULL	NULL	H3 Ab	GP		bind					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_2_225_s_117	10209020	(C)  ELISA of H3 Ab binding to the unphosphorylated H3 peptide  (open square), phosphorylated H3 peptide (closed square), total  cellular proteins from cycling cells (open circle) or from cells  treated with nocodazole (closed circle).	bind
54288	6	4404	6	NULL	NULL	NULL	NULL	H3 Ab	GP		bind					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_2_225_s_117	10209020	(C)  ELISA of H3 Ab binding to the unphosphorylated H3 peptide  (open square), phosphorylated H3 peptide (closed square), total  cellular proteins from cycling cells (open circle) or from cells  treated with nocodazole (closed circle).	bind
11038	1	4406	5	NULL	NULL	0	NULL	SEK1	NULL		bind	NULL				anti-SEK1 antibody	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_170_1_61_s_247	15998799	(C)  Immunoprecipitates were analyzed for SEK1 binding with anti-SEK1 or anti - rabbit  Akt antibody (top).	bind
11039	2	4406	5	NULL	NULL	0	NULL	SEK1	NULL		bind	NULL				anti - rabbit Akt antibody	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_170_1_61_s_247	15998799	(C)  Immunoprecipitates were analyzed for SEK1 binding with anti-SEK1 or anti - rabbit  Akt antibody (top).	bind
54289	1	4406	6	NULL	NULL	NULL	NULL	SEK1	GP		bind					anti-SEK1 antibody	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_170_1_61_s_247	15998799	(C)  Immunoprecipitates were analyzed for SEK1 binding with anti-SEK1 or anti - rabbit  Akt antibody (top).	bind
54290	2	4406	6	NULL	NULL	NULL	NULL	SEK1 	GP		bind					anti - rabbit Akt antibody	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_170_1_61_s_247	15998799	(C)  Immunoprecipitates were analyzed for SEK1 binding with anti-SEK1 or anti - rabbit  Akt antibody (top).	bind
11040	1	4407	5	NULL	NULL	0	NULL	DHFR-TS protein	NULL	plasmodium	bind	NULL	specifically			DHFR-TS RNA	NULL				NULL		0	NULL	NULL	NULL	gw60_science_296_5567_545_s_36	11964483	(C)  Plasmodium DHFR-TS protein bound  DHFR-TS RNA with specificity.	bind
10293	1	4407	6	NULL	NULL	NULL	NULL	DHFR-TS protein	GP	plasmodium	bind		specifically			DHFR-TS RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_science_296_5567_545_s_36	11964483	(C)  Plasmodium DHFR-TS protein bound  DHFR-TS RNA with specificity.	bind
11041	1	4408	5	NULL	NULL	0	NULL	Runx2	NULL		bind	NULL					NULL	mouse		A elements	NULL	hypertrophic MCT cells	0	NULL	NULL	NULL	gw70_cellbiol_162_5_833_s_108	12952936	(C)  Runx2 binds to the mouse A and B elements in hypertrophic MCT cells.	bind
11042	2	4408	5	NULL	NULL	0	NULL	Runx2	NULL		bind	NULL					NULL	mouse		B elements	NULL	hypertrophic MCT cells	0	NULL	NULL	NULL	gw70_cellbiol_162_5_833_s_108	12952936	(C)  Runx2 binds to the mouse A and B elements in hypertrophic MCT cells.	bind
10294	1	4408	6	NULL	NULL	NULL	NULL	Runx2	GP		bind							mouse		A element	NULL	hypertrophic MCT cells	NULL	NULL	NULL	NULL	gw70_cellbiol_162_5_833_s_108	12952936	(C)  Runx2 binds to the mouse A and B elements in hypertrophic MCT cells.	bind
10296	2	4408	6	NULL	NULL	NULL	NULL	Runx2	GP		bind							mouse		B element	NULL	hypertrophic MCT cells	NULL	NULL	NULL	NULL	gw70_cellbiol_162_5_833_s_108	12952936	(C)  Runx2 binds to the mouse A and B elements in hypertrophic MCT cells.	bind
11043	1	4409	5	NULL	NULL	0	NULL	syntaxin-1A	NULL		bind	NULL		191-240		myosin-Va	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_159	16030255	(C)  Syntaxin-1A [191-240] but not syntaxin-1A [191-240 L222] binds myosin-Va.	bind
11045	2	4409	5	NULL	NULL	0	NULL	syntaxin-1A	NULL		does not bind	NULL		191-240 L222		myosin-Va	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_159	16030255	(C)  Syntaxin-1A [191-240] but not syntaxin-1A [191-240 L222] binds myosin-Va.	bind
10297	1	4409	6	NULL	NULL	NULL	NULL	Syntaxin-1A	GP		bind			191-240		myosin-Va	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_159	16030255	(C)  Syntaxin-1A [191-240] but not syntaxin-1A [191-240 L222] binds myosin-Va.	bind
10298	2	4409	6	NULL	NULL	NULL	NULL	syntaxin-1A	GP		does not bind			191-240 L222		myosin-Va	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_159	16030255	(C)  Syntaxin-1A [191-240] but not syntaxin-1A [191-240 L222] binds myosin-Va.	bind
11048	1	4410	5	NULL	NULL	0	NULL	Sso	NULL		is not assembled into	NULL				SNARE complexes	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_8_3114_s_198	12925750	(C)  Vsm1 binds to Sso that is not assembled into  SNARE complexes.	bind
11049	2	4410	5	NULL	NULL	0	NULL	Vsm1	NULL		bind	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_8_3114_s_198	12925750	(C)  Vsm1 binds to Sso that is not assembled into  SNARE complexes.	bind
10300	2	4410	6	NULL	NULL	NULL	NULL	Vsm1	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_8_3114_s_198	12925750	(C)  Vsm1 binds to Sso that is not assembled into  SNARE complexes.	bind
10301	1	4410	6	NULL	NULL	NULL	NULL	Sso	GP		is not assembled into					SNARE complexes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_8_3114_s_198	12925750	(C)  Vsm1 binds to Sso that is not assembled into  SNARE complexes.	bind
11053	1	4413	5	NULL	NULL	0	NULL	PiC	NULL	35S-labeled	bind	NULL				Tom70	NULL	human	cytosolic segment (Hs-3)		NULL		0	NULL	NULL	NULL	gw60_cell_112_1_41_s_207	12526792	(C) 35S-labeled PiC (lane 1) was bound to human Tom70 cytosolic segment (Hs-3) and recovered with NiNTA-agarose as in	bind
10306	1	4413	6	NULL	NULL	NULL	NULL	PiC	GP	35S-labeled	bind					Tom70	GP	human	cytosolic segment (Hs-3)		NULL		NULL	NULL	NULL	NULL	gw60_cell_112_1_41_s_207	12526792	(C) 35S-labeled PiC (lane 1) was bound to human Tom70 cytosolic segment (Hs-3) and recovered with NiNTA-agarose as in	bind
11054	1	4414	5	NULL	NULL	0	NULL	GM1	NULL	3H-labeled	bind	NULL				CD1b	NULL	soluble			NULL		0	NULL	NULL	NULL	gw60_immunity_13_2_255_s_165	10981968	(C) 3H-labeled GM1 bound to soluble CD1b is displaced by cold GM2.	bind
11055	2	4414	5	NULL	NULL	0	NULL	GM2	NULL	cold	displaces	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_immunity_13_2_255_s_165	10981968	(C) 3H-labeled GM1 bound to soluble CD1b is displaced by cold GM2.	bind
10307	1	4414	6	NULL	NULL	NULL	NULL	GM1	GP	3H-labeled 	bind					CD1b	GP	soluble			NULL		NULL	NULL	NULL	NULL	gw60_immunity_13_2_255_s_165	10981968	(C) 3H-labeled GM1 bound to soluble CD1b is displaced by cold GM2.	bind
10309	2	4414	6	NULL	NULL	NULL	NULL	GM2	GP	cold	displaces					GM1	GP				NULL	statement 1	NULL	NULL	NULL	NULL	gw60_immunity_13_2_255_s_165	10981968	(C) 3H-labeled GM1 bound to soluble CD1b is displaced by cold GM2.	bind
11056	1	4415	5	NULL	NULL	0	NULL	PlexB	NULL		bind	NULL				RhoA	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_32_1_39_s_93	11604137	(C) A 40 amino acid deletion in PlexB  (PlexB d40) eliminates its binding to RhoA.	bind
11058	2	4415	5	NULL	NULL	0	NULL	PlexB d40	NULL		eliminate	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_32_1_39_s_93	11604137	(C) A 40 amino acid deletion in PlexB  (PlexB d40) eliminates its binding to RhoA.	bind
11059	3	4415	5	NULL	NULL	0	NULL	PlexB d40	NULL		is	NULL				40 amino acid deletion in PlexB	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_32_1_39_s_93	11604137	(C) A 40 amino acid deletion in PlexB  (PlexB d40) eliminates its binding to RhoA.	bind
10310	1	4415	6	NULL	NULL	NULL	NULL	PlexB	GP		bind					RhoA	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_1_39_s_93	11604137	(C) A 40 amino acid deletion in PlexB  (PlexB d40) eliminates its binding to RhoA.	bind
10311	2	4415	6	NULL	NULL	NULL	NULL	PlexBd40	GP		eliminates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_1_39_s_93	11604137	(C) A 40 amino acid deletion in PlexB  (PlexB d40) eliminates its binding to RhoA.	bind
54291	3	4415	6	NULL	NULL	NULL	NULL	PlexB d40	GP		is					40 amino acid deletion in PlexB	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_1_39_s_93	11604137	(C) A 40 amino acid deletion in PlexB  (PlexB d40) eliminates its binding to RhoA.	bind
11063	1	4417	5	NULL	NULL	0	NULL	EGFP-MuB	NULL		bind	NULL				target DNA molecules	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_10_6_1367_s_203	12504012	(C) A graph of the total fluorescence signal from the EGFP-MuB bound to the target DNA molecules versus time.	bind
10312	1	4417	6	NULL	NULL	NULL	NULL	EGFP-MuB	GP		bind					target DNA molecules	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_6_1367_s_203	12504012	(C) A graph of the total fluorescence signal from the EGFP-MuB bound to the target DNA molecules versus time.	bind
11065	1	4418	5	10	NULL	0	NULL	minichromosome		mardel derived;;human engineered	bind					CENP-A					NULL		NULL	NULL	NULL	NULL	gw60_devcell_1_2_165_s_20	11702777	(C) A mardel(10)-derived human engineered minichromosome (arrowed) (left panel; DAPI staining) binds CENP-A (red doublet signal; middle panel) and shows absence of  -satellite (yellow/green; right panel).	bind
10313	1	4418	6	NULL	NULL	NULL	NULL	minichromosome	Chromosome	mardel derived;;human engineered	bind					CENP-A	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_1_2_165_s_20	11702777	(C) A mardel(10)-derived human engineered minichromosome (arrowed) (left panel; DAPI staining) binds CENP-A (red doublet signal; middle panel) and shows absence of  -satellite (yellow/green; right panel).	bind
11069	1	4419	5	NULL	NULL	0	NULL	JM22z	NULL		bind	NULL				HLA-A2-flu	NULL				NULL		0	NULL	NULL	NULL	gw60_immunity_10_3_357_s_123	10204491	(C) A reaction profile illustrating the potential energy changes as JM22z binds to HLA-A2-flu.	bind
10317	1	4419	6	NULL	NULL	NULL	NULL	JM22z	GP		bind					HLA-A2-flu	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_10_3_357_s_123	10204491	(C) A reaction profile illustrating the potential energy changes as JM22z binds to HLA-A2-flu.	bind
11073	1	4421	5	10	NULL	0	NULL	P48 proteins		mutant;;human	heterodimerize with					E12					NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_117_s_276	16354684	(C) Ability of the mutant human P48 proteins to form heterodimers  with E12 and trimers with E12 and either RBP-J or RBP-L that bind the  Ela1 PTF1-site.	bind
11074	5	4421	5	10	NULL	0	NULL	P48 proteins		mutant;; human	form trimers with					 statement 2					NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_117_s_276	16354684	(C) Ability of the mutant human P48 proteins to form heterodimers  with E12 and trimers with E12 and either RBP-J or RBP-L that bind the  Ela1 PTF1-site.	bind
11075	4	4421	5	10	NULL	0	NULL	P48 proteins		mutant;;human	form trimers with					E12					NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_117_s_276	16354684	(C) Ability of the mutant human P48 proteins to form heterodimers  with E12 and trimers with E12 and either RBP-J or RBP-L that bind the  Ela1 PTF1-site.	bind
11077	6	4421	5	10	NULL	0	NULL	statement 4			occur simultaneously with					statement 5					NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_117_s_276	16354684	(C) Ability of the mutant human P48 proteins to form heterodimers  with E12 and trimers with E12 and either RBP-J or RBP-L that bind the  Ela1 PTF1-site.	bind
11078	3	4421	5	NULL	NULL	0	NULL	RBP-J	NULL		bind	NULL				Ela1	NULL			PTF1-site	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_117_s_276	16354684	(C) Ability of the mutant human P48 proteins to form heterodimers  with E12 and trimers with E12 and either RBP-J or RBP-L that bind the  Ela1 PTF1-site.	bind
11079	2	4421	5	NULL	NULL	0	NULL	RBP-L	NULL		bind	NULL				Ela1	NULL			PTF1-site	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_117_s_276	16354684	(C) Ability of the mutant human P48 proteins to form heterodimers  with E12 and trimers with E12 and either RBP-J or RBP-L that bind the  Ela1 PTF1-site.	bind
54293	7	4421	5	10	NULL	0	NULL	P48 proteins		human;;mutant	form trimers with					statement 3					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_1_117_s_276	16354684	(C) Ability of the mutant human P48 proteins to form heterodimers  with E12 and trimers with E12 and either RBP-J or RBP-L that bind the  Ela1 PTF1-site.	bind
54294	8	4421	5	10	NULL	0	NULL	statement 4			occur simultaneously with					statement 7					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_1_117_s_276	16354684	(C) Ability of the mutant human P48 proteins to form heterodimers  with E12 and trimers with E12 and either RBP-J or RBP-L that bind the  Ela1 PTF1-site.	bind
54295	9	4421	5	10	NULL	0	NULL	statement 6			is an alternative to					statement 8					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_1_117_s_276	16354684	(C) Ability of the mutant human P48 proteins to form heterodimers  with E12 and trimers with E12 and either RBP-J or RBP-L that bind the  Ela1 PTF1-site.	bind
10319	1	4421	6	NULL	NULL	NULL	NULL	P48 proteins	GP	mutant;; human	form heterodimers with					E12	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_117_s_276	16354684	(C) Ability of the mutant human P48 proteins to form heterodimers  with E12 and trimers with E12 and either RBP-J or RBP-L that bind the  Ela1 PTF1-site.	bind
10322	2	4421	6	NULL	NULL	NULL	NULL	RBP-J	GP		bind					Ela1	GP		PTF1-site		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_117_s_276	16354684	(C) Ability of the mutant human P48 proteins to form heterodimers  with E12 and trimers with E12 and either RBP-J or RBP-L that bind the  Ela1 PTF1-site.	bind
10324	3	4421	6	NULL	NULL	NULL	NULL	RBP-L	GP		bind					Ela1	GP		PTF1-site		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_117_s_276	16354684	(C) Ability of the mutant human P48 proteins to form heterodimers  with E12 and trimers with E12 and either RBP-J or RBP-L that bind the  Ela1 PTF1-site.	bind
10325	4	4421	6	NULL	NULL	NULL	NULL	P48 proteins	GP	mutant;;human	form trimers with					E12	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_117_s_276	16354684	(C) Ability of the mutant human P48 proteins to form heterodimers  with E12 and trimers with E12 and either RBP-J or RBP-L that bind the  Ela1 PTF1-site.	bind
12869	5	4421	6	NULL	NULL	NULL	NULL	P48 proteins	GP	mutant;;human	form trimers with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_117_s_276	16354684	(C) Ability of the mutant human P48 proteins to form heterodimers  with E12 and trimers with E12 and either RBP-J or RBP-L that bind the  Ela1 PTF1-site.	bind
12870	6	4421	6	NULL	NULL	NULL	NULL	statement 4	Process		occur simultaneously with					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_117_s_276	16354684	(C) Ability of the mutant human P48 proteins to form heterodimers  with E12 and trimers with E12 and either RBP-J or RBP-L that bind the  Ela1 PTF1-site.	bind
54296	7	4421	6	NULL	NULL	NULL	NULL	P48 proteins	GP	mutant;;human	form trimers with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_117_s_276	16354684	(C) Ability of the mutant human P48 proteins to form heterodimers  with E12 and trimers with E12 and either RBP-J or RBP-L that bind the  Ela1 PTF1-site.	bind
54297	8	4421	6	NULL	NULL	NULL	NULL	statement 4	Process		occur simultaneously with					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_117_s_276	16354684	(C) Ability of the mutant human P48 proteins to form heterodimers  with E12 and trimers with E12 and either RBP-J or RBP-L that bind the  Ela1 PTF1-site.	bind
54298	9	4421	6	NULL	NULL	NULL	NULL	statement 6	Process		is an alternative to					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_117_s_276	16354684	(C) Ability of the mutant human P48 proteins to form heterodimers  with E12 and trimers with E12 and either RBP-J or RBP-L that bind the  Ela1 PTF1-site.	bind
11080	1	4424	5	NULL	NULL	0	NULL	cortactin	NULL	mutant	does not bind	NULL		W22A		Arp2/3 complex	NULL				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_21_1852_s_28	12419186	(C) Actin dynamics in cells expressing mutant forms of cortactin that do not bind Arp2/3 complex (cortactin W22A) or dynamin2 (cortactin W525K).	bind
11081	2	4424	5	NULL	NULL	0	NULL	cortactin	NULL	mutant	does not bind	NULL		W525K		dynamin2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_21_1852_s_28	12419186	(C) Actin dynamics in cells expressing mutant forms of cortactin that do not bind Arp2/3 complex (cortactin W22A) or dynamin2 (cortactin W525K).	bind
10326	1	4424	6	NULL	NULL	NULL	NULL	cortactin	GP	mutant	does not bind			W22A		Arp2/3 complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_21_1852_s_28	12419186	(C) Actin dynamics in cells expressing mutant forms of cortactin that do not bind Arp2/3 complex (cortactin W22A) or dynamin2 (cortactin W525K).	bind
10327	2	4424	6	NULL	NULL	NULL	NULL	cortactin	GP	mutant	does not bind			W525K		dynamin2	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_21_1852_s_28	12419186	(C) Actin dynamics in cells expressing mutant forms of cortactin that do not bind Arp2/3 complex (cortactin W22A) or dynamin2 (cortactin W525K).	bind
11082	1	4425	5	NULL	NULL	0	NULL	Adf-1	NULL		bind	NULL				TAFII110	NULL				NULL	in vivo	0	NULL	NULL	NULL	gw60_molcellbiol_18_4_2252_s_269	9528796	(C) Adf-1 binds the same regions of TAFII110 and TAFII250 in vivo as it does in vitro.	bind
11083	2	4425	5	NULL	NULL	0	NULL	Adf-1	NULL		bind	NULL				TAFII250	NULL				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2252_s_269	9528796	(C) Adf-1 binds the same regions of TAFII110 and TAFII250 in vivo as it does in vitro.	bind
11084	3	4425	5	NULL	NULL	0	NULL	Adf-1	NULL		bind	NULL				TAFII110	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_molcellbiol_18_4_2252_s_269	9528796	(C) Adf-1 binds the same regions of TAFII110 and TAFII250 in vivo as it does in vitro.	bind
11085	4	4425	5	NULL	NULL	0	NULL	Adf-1	NULL		bind	NULL				TAFII250	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_molcellbiol_18_4_2252_s_269	9528796	(C) Adf-1 binds the same regions of TAFII110 and TAFII250 in vivo as it does in vitro.	bind
10328	1	4425	6	NULL	NULL	NULL	NULL	Adf-1	GP		bind					TAFII110	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2252_s_269	9528796	(C) Adf-1 binds the same regions of TAFII110 and TAFII250 in vivo as it does in vitro.	bind
10329	2	4425	6	NULL	NULL	NULL	NULL	Adf-1	GP		bind					TAFII250	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2252_s_269	9528796	(C) Adf-1 binds the same regions of TAFII110 and TAFII250 in vivo as it does in vitro.	bind
10330	3	4425	6	NULL	NULL	NULL	NULL	Adf-1	GP		bind					TAFII250	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2252_s_269	9528796	(C) Adf-1 binds the same regions of TAFII110 and TAFII250 in vivo as it does in vitro.	bind
10331	4	4425	6	NULL	NULL	NULL	NULL	Adf-1	GP		bind					TAFII110	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2252_s_269	9528796	(C) Adf-1 binds the same regions of TAFII110 and TAFII250 in vivo as it does in vitro.	bind
11086	1	4426	5	NULL	NULL	0	NULL	p53	NULL		bind	NULL				Snk/Plk2	NULL			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_16_5556_s_203	12897130	(c) Adriamycin treatment enhances p53 binding  to the Snk/Plk2 promoter in vivo.	bind
11087	2	4426	5	NULL	NULL	0	NULL	Adriamycin	NULL	treatment of	enhances	NULL				statement 1	NULL				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_16_5556_s_203	12897130	(c) Adriamycin treatment enhances p53 binding  to the Snk/Plk2 promoter in vivo.	bind
10332	1	4426	6	NULL	NULL	NULL	NULL	p53	GP		bind					Snk/Plk2	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_16_5556_s_203	12897130	(c) Adriamycin treatment enhances p53 binding  to the Snk/Plk2 promoter in vivo.	bind
10333	2	4426	6	NULL	NULL	NULL	NULL	adriamycin	Chemical	treatment of	enhances					statement 1	Process				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_16_5556_s_203	12897130	(c) Adriamycin treatment enhances p53 binding  to the Snk/Plk2 promoter in vivo.	bind
11215	1	4428	5	10	NULL	0	NULL	GST-SOX9	NULL		bind	NULL				AMH	NULL			SOX-BS in proximal promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_11_6653_s_185	9774680	(C) Affinity binding of GST-SOX9 to the SOX-binding site (SOX-BS) in the AMH proximal promoter probe.	bind
11216	2	4428	5	NULL	NULL	0	NULL	SOX-BS	NULL		is	NULL				SOX-binding site	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_11_6653_s_185	9774680	(C) Affinity binding of GST-SOX9 to the SOX-binding site (SOX-BS) in the AMH proximal promoter probe.	bind
10334	1	4428	6	NULL	NULL	NULL	NULL	GST-SOX9	GP		bind					AMH 	GP			SOX-BS in the proximal promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_11_6653_s_185	9774680	(C) Affinity binding of GST-SOX9 to the SOX-binding site (SOX-BS) in the AMH proximal promoter probe.	bind
10335	2	4428	6	NULL	NULL	NULL	NULL	SOX-BS			is					SOX-binding site					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_11_6653_s_185	9774680	(C) Affinity binding of GST-SOX9 to the SOX-binding site (SOX-BS) in the AMH proximal promoter probe.	bind
11217	1	4431	5	NULL	NULL	0	NULL	SOS	NULL	Drosophila	bind	NULL	strongly			Drk	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_6_1_65_s_234	10949028	(C) Alignment of the C terminus of ARK-1 with a region of  Drosophila SOS that binds strongly to Drk, the  Drosophila ortholog of SEM-5 (see  Raabe et al. 1995  ).	bind
13122	2	4431	5	10	NULL	0	NULL	Drk		Drosophila	is ortholog of					SEM-5					NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_1_65_s_234	10949028	(C) Alignment of the C terminus of ARK-1 with a region of  Drosophila SOS that binds strongly to Drk, the  Drosophila ortholog of SEM-5 (see  Raabe et al. 1995  ).	bind
10337	1	4431	6	NULL	NULL	NULL	NULL	SOS	GP	Drosophila	bind		strongly			Drk	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_1_65_s_234	10949028	(C) Alignment of the C terminus of ARK-1 with a region of  Drosophila SOS that binds strongly to Drk, the  Drosophila ortholog of SEM-5 (see  Raabe et al. 1995  ).	bind
10338	2	4431	6	NULL	NULL	NULL	NULL	Drk	GP	Drosophila	is ortholog of					SEM-5	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_1_65_s_234	10949028	(C) Alignment of the C terminus of ARK-1 with a region of  Drosophila SOS that binds strongly to Drk, the  Drosophila ortholog of SEM-5 (see  Raabe et al. 1995  ).	bind
11220	1	4436	5	NULL	NULL	0	NULL	Ets2-Fli1 fusion protein	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_7_2467_s_232	16537893	(C) An Ets2-Fli1 fusion protein binds DNA cooperatively  with Fos-Jun.	bind
11222	2	4436	5	NULL	NULL	0	NULL	Fos-Jun	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_7_2467_s_232	16537893	(C) An Ets2-Fli1 fusion protein binds DNA cooperatively  with Fos-Jun.	bind
11223	3	4436	5	NULL	NULL	0	NULL	statement 1	NULL		occurs in cooperation with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_7_2467_s_232	16537893	(C) An Ets2-Fli1 fusion protein binds DNA cooperatively  with Fos-Jun.	bind
10339	1	4436	6	NULL	NULL	NULL	NULL	 Ets2-Fli1	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_7_2467_s_232	16537893	(C) An Ets2-Fli1 fusion protein binds DNA cooperatively  with Fos-Jun.	bind
10340	2	4436	6	NULL	NULL	NULL	NULL	Fos-Jun	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_7_2467_s_232	16537893	(C) An Ets2-Fli1 fusion protein binds DNA cooperatively  with Fos-Jun.	bind
12785	3	4436	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_7_2467_s_232	16537893	(C) An Ets2-Fli1 fusion protein binds DNA cooperatively  with Fos-Jun.	bind
11224	1	4437	5	10	NULL	0	NULL	anti-VCP IgY 		affinity-purified	bind					rVCP					NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_30_s_115	12922167	(c) Analysis of affinity-purified anti-VCP IgY (primary antibody) binding to rVCP, and anti-chicken IgG (secondary antibody) binding to anti-VCP IgY primary antibody.	bind
11225	2	4437	5	10	NULL	0	NULL	anti-chicken IgG 			bind					anti-VCP IgY 					NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_30_s_115	12922167	(c) Analysis of affinity-purified anti-VCP IgY (primary antibody) binding to rVCP, and anti-chicken IgG (secondary antibody) binding to anti-VCP IgY primary antibody.	bind
54299	3	4437	5	10	NULL	0	NULL	anti-VCP IgY			is a type of					primary antibody					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_30_s_115	12922167	(c) Analysis of affinity-purified anti-VCP IgY (primary antibody) binding to rVCP, and anti-chicken IgG (secondary antibody) binding to anti-VCP IgY primary antibody.	bind
54300	4	4437	5	10	NULL	0	NULL	anti-chicken IgG 			is a type of					secondary antibody					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_30_s_115	12922167	(c) Analysis of affinity-purified anti-VCP IgY (primary antibody) binding to rVCP, and anti-chicken IgG (secondary antibody) binding to anti-VCP IgY primary antibody.	bind
10341	1	4437	6	NULL	NULL	NULL	NULL	anti-VCP IgY	GP	affinity-purified	bind					rVCP	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_30_s_115	12922167	(c) Analysis of affinity-purified anti-VCP IgY (primary antibody) binding to rVCP, and anti-chicken IgG (secondary antibody) binding to anti-VCP IgY primary antibody.	bind
10342	2	4437	6	NULL	NULL	NULL	NULL	anti-chicken IgG	GP		bind					anti-VCP IgY 	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_30_s_115	12922167	(c) Analysis of affinity-purified anti-VCP IgY (primary antibody) binding to rVCP, and anti-chicken IgG (secondary antibody) binding to anti-VCP IgY primary antibody.	bind
54301	3	4437	6	NULL	NULL	NULL	NULL	anti-VCP IgY	GP		is a type of					primary antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_30_s_115	12922167	(c) Analysis of affinity-purified anti-VCP IgY (primary antibody) binding to rVCP, and anti-chicken IgG (secondary antibody) binding to anti-VCP IgY primary antibody.	bind
54302	4	4437	6	NULL	NULL	NULL	NULL	anti-chicken IgG	GP		is a type of					secondary antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_30_s_115	12922167	(c) Analysis of affinity-purified anti-VCP IgY (primary antibody) binding to rVCP, and anti-chicken IgG (secondary antibody) binding to anti-VCP IgY primary antibody.	bind
11227	1	4438	5	10	NULL	0	NULL	eIF2		purified	bind					eIF2B complex		FLAG-tagged;; wild-type			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_11_3965_s_323	10805739	(C) Analysis of binding between the indicated concentration of purified eIF2 and FLAG-tagged wild-type eIF2B complex (lanes 7 to 10) or eIF2BepsilonF250L (lanes 11 to 14).	bind
11228	2	4438	5	NULL	NULL	0	NULL	eIF2	NULL	purified	bind	NULL				eIF2Bepsilon	NULL		F250L		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_11_3965_s_323	10805739	(C) Analysis of binding between the indicated concentration of purified eIF2 and FLAG-tagged wild-type eIF2B complex (lanes 7 to 10) or eIF2BepsilonF250L (lanes 11 to 14).	bind
54303	3	4438	5	10	NULL	0	NULL	statement 1			is an alternative to					statement 2					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_11_3965_s_323	10805739	(C) Analysis of binding between the indicated concentration of purified eIF2 and FLAG-tagged wild-type eIF2B complex (lanes 7 to 10) or eIF2BepsilonF250L (lanes 11 to 14).	bind
10523	1	4438	6	NULL	NULL	NULL	NULL	eIF2	GP		bind					eIF2B complex	GP	FLAG-tagged;;wild type			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_11_3965_s_323	10805739	(C) Analysis of binding between the indicated concentration of purified eIF2 and FLAG-tagged wild-type eIF2B complex (lanes 7 to 10) or eIF2BepsilonF250L (lanes 11 to 14).	bind
10524	2	4438	6	NULL	NULL	NULL	NULL	eIF2	GP		bind					eIF2Bepsilon	GP		F250L		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_11_3965_s_323	10805739	(C) Analysis of binding between the indicated concentration of purified eIF2 and FLAG-tagged wild-type eIF2B complex (lanes 7 to 10) or eIF2BepsilonF250L (lanes 11 to 14).	bind
10525	3	4438	6	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_11_3965_s_323	10805739	(C) Analysis of binding between the indicated concentration of purified eIF2 and FLAG-tagged wild-type eIF2B complex (lanes 7 to 10) or eIF2BepsilonF250L (lanes 11 to 14).	bind
11230	1	4439	5	NULL	NULL	0	NULL	NFATp/c	NULL		bind	NULL					NULL			IL190 element	NULL	PMA/I-activated Jurkat cell nuclear extracts	0	NULL	NULL	NULL	gw60_immunity_6_2_175_s_150	9047239	(C) Analysis of NFATp/c and Oct binding to the IL190 element using PMA/I-activated Jurkat cell nuclear extracts in the presence and absence of 1  l of Oct-1 and 0.2  l of NFATp antisera.	bind
11231	2	4439	5	NULL	NULL	0	NULL	Oct	NULL		bind	NULL					NULL			IL190 element	NULL	PMA/I-activated Jurkat cell nuclear extracts 	0	NULL	NULL	NULL	gw60_immunity_6_2_175_s_150	9047239	(C) Analysis of NFATp/c and Oct binding to the IL190 element using PMA/I-activated Jurkat cell nuclear extracts in the presence and absence of 1  l of Oct-1 and 0.2  l of NFATp antisera.	bind
10529	1	4439	6	NULL	NULL	NULL	NULL	NFATp/c	GP		bind									IL190 element	NULL	PMA/I-activated Jurkat cell nuclear extracts	NULL	NULL	NULL	NULL	gw60_immunity_6_2_175_s_150	9047239	(C) Analysis of NFATp/c and Oct binding to the IL190 element using PMA/I-activated Jurkat cell nuclear extracts in the presence and absence of 1  l of Oct-1 and 0.2  l of NFATp antisera.	bind
10531	2	4439	6	NULL	NULL	NULL	NULL	Oct	GP		bind									IL190 element	NULL	PMA/I-activated Jurkat cell nuclear extracts	NULL	NULL	NULL	NULL	gw60_immunity_6_2_175_s_150	9047239	(C) Analysis of NFATp/c and Oct binding to the IL190 element using PMA/I-activated Jurkat cell nuclear extracts in the presence and absence of 1  l of Oct-1 and 0.2  l of NFATp antisera.	bind
11232	1	4440	5	10	NULL	0	NULL				bind			E-NTD 		RseA-cyto-His6					NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_4_1067_s_148	12718891	(C) Anti- E Western blot showing that both  E-NTD and -CTD domains bind to RseA-cyto-His6.	bind
11233	2	4440	5	10	NULL	0	NULL				bind			E-CTD		RseA-cyto-His6					NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_4_1067_s_148	12718891	(C) Anti- E Western blot showing that both  E-NTD and -CTD domains bind to RseA-cyto-His6.	bind
10535	1	4440	6	NULL	NULL	NULL	NULL				bind			E-NTD		RseA-cyto-His6	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_4_1067_s_148	12718891	(C) Anti- E Western blot showing that both  E-NTD and -CTD domains bind to RseA-cyto-His6.	bind
10536	2	4440	6	NULL	NULL	NULL	NULL				bind			E-CTD		RseA-cyto-His6	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_4_1067_s_148	12718891	(C) Anti- E Western blot showing that both  E-NTD and -CTD domains bind to RseA-cyto-His6.	bind
11234	1	4441	5	NULL	NULL	0	NULL	AP-1	NULL		bind	NULL				normal membranes	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_cell_114_3_299_s_170	12914695	(C) Anti-PI(4)P blocks AP-1 binding to normal membranes in vitro.	bind
11235	2	4441	5	NULL	NULL	0	NULL	anti-PI(4)P	NULL		blocks	NULL				statement 1	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_cell_114_3_299_s_170	12914695	(C) Anti-PI(4)P blocks AP-1 binding to normal membranes in vitro.	bind
10537	1	4441	6	NULL	NULL	NULL	NULL	AP-1	GP		bind					normal membranes	CellComponent				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_cell_114_3_299_s_170	12914695	(C) Anti-PI(4)P blocks AP-1 binding to normal membranes in vitro.	bind
10538	2	4441	6	NULL	NULL	NULL	NULL	Anti-PI(4)P	GP		blocks					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_cell_114_3_299_s_170	12914695	(C) Anti-PI(4)P blocks AP-1 binding to normal membranes in vitro.	bind
11237	1	4442	5	NULL	NULL	0	NULL	PF2 antibody	NULL		bind	NULL				zonular microfibrils 	NULL	bovine			NULL	middle of the interbead 	NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_1045_s_156	11238459	(C) Antibody PF2 (purple) binds bovine zonular microfibrils near the middle of the interbead.	bind
10539	1	4442	6	NULL	NULL	NULL	NULL	PF2 antibody	GP		bind					zonular microfibrils	CellComponent	bovine			NULL	middle of the interbead	NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_1045_s_156	11238459	(C) Antibody PF2 (purple) binds bovine zonular microfibrils near the middle of the interbead.	bind
11238	1	4443	5	NULL	NULL	0	NULL	AP-2	NULL		bind	NULL				C40 enhancer	NULL			AP-2(B) motif in	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_8_3308_s_272	16581802	(C) AP-2 binds to the AP-2(B) motif within the C40 enhancer.	bind
10540	1	4443	6	NULL	NULL	NULL	NULL	AP-2	GP		bind					C40 enhancer	GP			AP-2(B) motif in	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_8_3308_s_272	16581802	(C) AP-2 binds to the AP-2(B) motif within the C40 enhancer.	bind
11241	1	4444	5	NULL	NULL	0	NULL	APA-1	NULL		bind	NULL				MMP1	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_21_7385_s_321	12370286	(C) APA-1 binds to the  MMP1 promoter.	bind
10541	1	4444	6	NULL	NULL	NULL	NULL	APA-1	GP		bind					MMP1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_21_7385_s_321	12370286	(C) APA-1 binds to the  MMP1 promoter.	bind
11242	1	4445	5	10	NULL	0	NULL	ArpA			does not bind			W119A		A-factor					NULL		NULL	NULL	NULL	NULL	gw60_gene_222_1_133_s_210	9813285	(c) ArpA/W119A does not bind A-factor, since almost no radioactivity elutes in fractions 3 and 4 in either the presence ( ) or the absence ( ) of non-labelled A-factor.	bind
10542	1	4445	6	NULL	NULL	NULL	NULL	ArpA	GP		does not bind			W119A		A-factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_gene_222_1_133_s_210	9813285	(c) ArpA/W119A does not bind A-factor, since almost no radioactivity elutes in fractions 3 and 4 in either the presence ( ) or the absence ( ) of non-labelled A-factor.	bind
11245	1	4446	5	NULL	NULL	0	NULL	Hsp70/Hsc70	NULL	endogenous	bind	NULL				GADD34-BAG-1 complex	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_10_3477_s_145	12724406	(C) ATP modulation of the binding of endogenous Hsp70/Hsc70 and PP1 to the GADD34-BAG-1 complex.	bind
11247	2	4446	5	NULL	NULL	0	NULL	PP1	NULL	endogenous	bind	NULL				GADD34-BAG-1 complex	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_10_3477_s_145	12724406	(C) ATP modulation of the binding of endogenous Hsp70/Hsc70 and PP1 to the GADD34-BAG-1 complex.	bind
11248	3	4446	5	NULL	NULL	0	NULL	ATP	NULL		modulate	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_10_3477_s_145	12724406	(C) ATP modulation of the binding of endogenous Hsp70/Hsc70 and PP1 to the GADD34-BAG-1 complex.	bind
11249	4	4446	5	NULL	NULL	0	NULL	ATP	NULL		modulate	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_10_3477_s_145	12724406	(C) ATP modulation of the binding of endogenous Hsp70/Hsc70 and PP1 to the GADD34-BAG-1 complex.	bind
10543	1	4446	6	NULL	NULL	NULL	NULL	Hsp70/Hsc70	GP	endogenous	bind					GADD34-BAG-1 complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_10_3477_s_145	12724406	(C) ATP modulation of the binding of endogenous Hsp70/Hsc70 and PP1 to the GADD34-BAG-1 complex.	bind
10544	2	4446	6	NULL	NULL	NULL	NULL	PP1	GP	endogenous	bind					GADD34-BAG-1 complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_10_3477_s_145	12724406	(C) ATP modulation of the binding of endogenous Hsp70/Hsc70 and PP1 to the GADD34-BAG-1 complex.	bind
12786	3	4446	6	NULL	NULL	NULL	NULL	ATP	Chemical		modulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_10_3477_s_145	12724406	(C) ATP modulation of the binding of endogenous Hsp70/Hsc70 and PP1 to the GADD34-BAG-1 complex.	bind
12787	4	4446	6	NULL	NULL	NULL	NULL	ATP	Chemical		modulates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_10_3477_s_145	12724406	(C) ATP modulation of the binding of endogenous Hsp70/Hsc70 and PP1 to the GADD34-BAG-1 complex.	bind
11250	1	4447	5	NULL	NULL	0	NULL	CAND1	NULL		bind	NULL				CUL1	NULL				NULL	HeLa extracts	0	NULL	NULL	NULL	gw60_molcell_10_6_1519_s_135	12504026	(C) ATP prevents the binding of CAND1 to CUL1 in HeLa extracts.	bind
11251	2	4447	5	NULL	NULL	0	NULL	ATP	NULL		prevent	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_10_6_1519_s_135	12504026	(C) ATP prevents the binding of CAND1 to CUL1 in HeLa extracts.	bind
10545	1	4447	6	NULL	NULL	NULL	NULL	CAND1	GP		bind					CUL1	GP				NULL	HeLa nuclear extracts	NULL	NULL	NULL	NULL	gw60_molcell_10_6_1519_s_135	12504026	(C) ATP prevents the binding of CAND1 to CUL1 in HeLa extracts.	bind
10546	2	4447	6	NULL	NULL	NULL	NULL	ATP	Chemical		prevents					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_6_1519_s_135	12504026	(C) ATP prevents the binding of CAND1 to CUL1 in HeLa extracts.	bind
11253	1	4448	5	NULL	NULL	0	NULL	Aurora-A	NULL		bind	NULL				CNN	NULL		COOH-terminal domain		NULL		0	NULL	NULL	NULL	gw70_cellbiol_162_5_757_s_32	12939255	(C) Aurora-A  binds to the COOH-terminal domain of CNN.	bind
10547	1	4448	6	NULL	NULL	NULL	NULL	Aurora-A	GP		bind					CNN	GP		COOH-terminal domain		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_162_5_757_s_32	12939255	(C) Aurora-A  binds to the COOH-terminal domain of CNN.	bind
11255	1	4449	5	NULL	NULL	0	NULL	PAPs	NULL	35S-labeled	bind	NULL				GST-cyclin B1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_14_5310_s_133	10866687	(C) Autoradiogram of 35S-labeled PAPs bound to either GST-cyclin B1 (lanes 1, 3, 5, and 7) or GST (lanes 2, 4, 6, and 8).	bind
11256	2	4449	5	NULL	NULL	0	NULL	PAPs	NULL	35S-labeled	bind	NULL				GST	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_14_5310_s_133	10866687	(C) Autoradiogram of 35S-labeled PAPs bound to either GST-cyclin B1 (lanes 1, 3, 5, and 7) or GST (lanes 2, 4, 6, and 8).	bind
13123	3	4449	5	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_14_5310_s_133	10866687	(C) Autoradiogram of 35S-labeled PAPs bound to either GST-cyclin B1 (lanes 1, 3, 5, and 7) or GST (lanes 2, 4, 6, and 8).	bind
10548	1	4449	6	NULL	NULL	NULL	NULL	PAPs	GP	35S-labeled	bind					GST-cyclin B1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_14_5310_s_133	10866687	(C) Autoradiogram of 35S-labeled PAPs bound to either GST-cyclin B1 (lanes 1, 3, 5, and 7) or GST (lanes 2, 4, 6, and 8).	bind
10549	2	4449	6	NULL	NULL	NULL	NULL	PAPs	GP	35S-labeled	bind					GST					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_14_5310_s_133	10866687	(C) Autoradiogram of 35S-labeled PAPs bound to either GST-cyclin B1 (lanes 1, 3, 5, and 7) or GST (lanes 2, 4, 6, and 8).	bind
10550	3	4449	6	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_14_5310_s_133	10866687	(C) Autoradiogram of 35S-labeled PAPs bound to either GST-cyclin B1 (lanes 1, 3, 5, and 7) or GST (lanes 2, 4, 6, and 8).	bind
11257	1	4450	5	10	NULL	0	NULL	hybrid 8			bind					32P DNA					NULL		NULL	NULL	NULL	NULL	gw60_chembiol_10_8_713_s_142	12954330	(C) Autoradiogram showing the binding of hybrid  8 to 32P DNAs (45 pM).	bind
10551	1	4450	6	NULL	NULL	NULL	NULL	hybrid 8			bind					32P DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_10_8_713_s_142	12954330	(C) Autoradiogram showing the binding of hybrid  8 to 32P DNAs (45 pM).	bind
11258	1	4453	5	NULL	NULL	0	NULL	PriA protein	NULL		bind	NULL				Fork 4	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_9_2_241_s_197	11864599	(C) Band-shift assay showing binding of PriA and SrgA proteins to Fork 4 in the presence of EDTA.	bind
11259	2	4453	5	NULL	NULL	0	NULL	statement 1	NULL		in the presence of	NULL				EDTA	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_9_2_241_s_197	11864599	(C) Band-shift assay showing binding of PriA and SrgA proteins to Fork 4 in the presence of EDTA.	bind
11260	3	4453	5	NULL	NULL	0	NULL	SrgA protein	NULL		bind	NULL				Fork 4	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_9_2_241_s_197	11864599	(C) Band-shift assay showing binding of PriA and SrgA proteins to Fork 4 in the presence of EDTA.	bind
11261	4	4453	5	NULL	NULL	0	NULL	statement 3	NULL		in the presence of	NULL				EDTA	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_9_2_241_s_197	11864599	(C) Band-shift assay showing binding of PriA and SrgA proteins to Fork 4 in the presence of EDTA.	bind
10552	1	4453	6	NULL	NULL	NULL	NULL	PriA	GP		bind					Fork 4	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_9_2_241_s_197	11864599	(C) Band-shift assay showing binding of PriA and SrgA proteins to Fork 4 in the presence of EDTA.	bind
10553	2	4453	6	NULL	NULL	NULL	NULL	SrgA	GP		bind					Fork 4	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_9_2_241_s_197	11864599	(C) Band-shift assay showing binding of PriA and SrgA proteins to Fork 4 in the presence of EDTA.	bind
10554	3	4453	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs in presence of					EDTA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_9_2_241_s_197	11864599	(C) Band-shift assay showing binding of PriA and SrgA proteins to Fork 4 in the presence of EDTA.	bind
10555	4	4453	6	NULL	NULL	NULL	NULL	statement 2	Process		occurs in presence of					EDTA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_9_2_241_s_197	11864599	(C) Band-shift assay showing binding of PriA and SrgA proteins to Fork 4 in the presence of EDTA.	bind
11263	1	4454	5	NULL	NULL	0	NULL	NR	NULL		bind	NULL					NULL		RBD-2		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_203	10891484	(C) Basic/polar residues N terminal to the core LXXLL motif are critical for NR binding to RBD-2.	bind
11264	2	4454	5	NULL	NULL	0	NULL		NULL		critical for	NULL		basic/polar residues N terminal to core LXXLL motif		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_203	10891484	(C) Basic/polar residues N terminal to the core LXXLL motif are critical for NR binding to RBD-2.	bind
10761	1	4454	6	NULL	NULL	NULL	NULL	NR	GP		bind								RBD-2		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_203	10891484	(C) Basic/polar residues N terminal to the core LXXLL motif are critical for NR binding to RBD-2.	bind
10762	2	4454	6	NULL	NULL	NULL	NULL				are critical for			Basic/polar residues N terminal to the core LXXLL motif		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_203	10891484	(C) Basic/polar residues N terminal to the core LXXLL motif are critical for NR binding to RBD-2.	bind
11267	1	4455	5	NULL	NULL	0	NULL	Bcl-3 protein	NULL		bind	NULL				cyclin D1	NULL			proximal NF-kappaB site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_24_8428_s_190	11713278	(C) Bcl-3 and p52 proteins bind to the proximal NF-kappaB site of the cyclin D1 promoter.	bind
11268	2	4455	5	NULL	NULL	0	NULL	p52 protein	NULL		bind	NULL				cyclin D1	NULL			proximal NF-kappaB site of promoter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_24_8428_s_190	11713278	(C) Bcl-3 and p52 proteins bind to the proximal NF-kappaB site of the cyclin D1 promoter.	bind
10763	1	4455	6	NULL	NULL	NULL	NULL	Bcl-3	GP		bind					cyclin D1	GP			proximal NF-kappaB site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_24_8428_s_190	11713278	(C) Bcl-3 and p52 proteins bind to the proximal NF-kappaB site of the cyclin D1 promoter.	bind
10764	2	4455	6	NULL	NULL	NULL	NULL	p52	GP		bind					cyclin D1	GP			proximal NF-kappaB site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_24_8428_s_190	11713278	(C) Bcl-3 and p52 proteins bind to the proximal NF-kappaB site of the cyclin D1 promoter.	bind
11270	1	4457	5	NULL	NULL	0	NULL	BCS1(84-126)-DHFR	NULL		bind	NULL				OMV	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_7_2239_s_277	12640110	(C) BCS1(84-126)-DHFR bound to OMV can be coimmunoprecipitated  with components of the TOM complex.	bind
11272	2	4457	5	NULL	NULL	0	NULL	statement 1	NULL		coimmunoprecipitates with	NULL				TOM complex	NULL	components of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_7_2239_s_277	12640110	(C) BCS1(84-126)-DHFR bound to OMV can be coimmunoprecipitated  with components of the TOM complex.	bind
10765	1	4457	6	NULL	NULL	NULL	NULL	BCS1-DHFR	GP		bind					OMV	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_7_2239_s_277	12640110	(C) BCS1(84-126)-DHFR bound to OMV can be coimmunoprecipitated  with components of the TOM complex.	bind
10766	2	4457	6	NULL	NULL	NULL	NULL	statement 1	Process		coimmunoprecipitates					TOM complex	CellComponent	components of 			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_7_2239_s_277	12640110	(C) BCS1(84-126)-DHFR bound to OMV can be coimmunoprecipitated  with components of the TOM complex.	bind
11274	1	4460	5	NULL	NULL	0	NULL	Bfa1p	NULL		bind	NULL	directly			Cdc14p	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_157_3_367_s_102	11970961	(C) Bfa1p and Tem1p bind directly to Cdc14p.	bind
11275	2	4460	5	NULL	NULL	0	NULL	Tem1p	NULL		bind	NULL	directly			Cdc14p	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_157_3_367_s_102	11970961	(C) Bfa1p and Tem1p bind directly to Cdc14p.	bind
10767	1	4460	6	NULL	NULL	NULL	NULL	Bfa1p	GP		bind		directly			Cdc14p	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_3_367_s_102	11970961	(C) Bfa1p and Tem1p bind directly to Cdc14p.	bind
10768	2	4460	6	NULL	NULL	NULL	NULL	Tem1p	GP		bind		directly			Cdc14p	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_3_367_s_102	11970961	(C) Bfa1p and Tem1p bind directly to Cdc14p.	bind
11277	1	4461	5	NULL	NULL	0	NULL	CRMP-2	NULL		bind	NULL				tubulin	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_22_9973_s_149	16260611	(C) Biacore sensorgram of CRMP-2 binding to tubulin.	bind
10769	1	4461	6	NULL	NULL	NULL	NULL	CRMP-2	GP		bind					tubulin	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9973_s_149	16260611	(C) Biacore sensorgram of CRMP-2 binding to tubulin.	bind
11278	1	4462	5	NULL	NULL	0	NULL	wtBH3	NULL		is	NULL				Bim BH3 peptide	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_162_5_877_s_100	12952938	(C) Bim BH3 peptide (wtBH3) binds Bcl-w as well as BimLdeltaC27.	bind
11280	2	4462	5	NULL	NULL	0	NULL	wtBH3	NULL		bind	NULL				Bcl-w	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_162_5_877_s_100	12952938	(C) Bim BH3 peptide (wtBH3) binds Bcl-w as well as BimLdeltaC27.	bind
11282	3	4462	5	10	NULL	0	NULL	wtBH3			bind					BimLdeltaC27					NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_162_5_877_s_100	12952938	(C) Bim BH3 peptide (wtBH3) binds Bcl-w as well as BimLdeltaC27.	bind
10770	1	4462	6	NULL	NULL	NULL	NULL	Bim BH3 peptide	AminoAcid	wild type	bind					Bcl-w	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_162_5_877_s_100	12952938	(C) Bim BH3 peptide (wtBH3) binds Bcl-w as well as BimLdeltaC27.	bind
10771	2	4462	6	NULL	NULL	NULL	NULL	Bim BH3 peptide	AminoAcid	wild type	bind					BimLdeltaC27	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_162_5_877_s_100	12952938	(C) Bim BH3 peptide (wtBH3) binds Bcl-w as well as BimLdeltaC27.	bind
54304	3	4462	6	NULL	NULL	NULL	NULL	wtBH3	GP		is					Bim BH3 peptide	AminoAcid	wild type			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_162_5_877_s_100	12952938	(C) Bim BH3 peptide (wtBH3) binds Bcl-w as well as BimLdeltaC27.	bind
11284	1	4463	5	NULL	NULL	0	NULL	IgG2 MAbs	NULL		bind	NULL				PNAG antigen	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_74_5_2742_s_161	16622211	(C) Binding  of IgG2 MAbs to PNAG antigen.	bind
10772	1	4463	6	NULL	NULL	NULL	NULL	IgG2 MAbs	GP		bind					PNAG antigen	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_74_5_2742_s_161	16622211	(C) Binding  of IgG2 MAbs to PNAG antigen.	bind
11285	1	4464	5	NULL	NULL	0	NULL	MECA-79 antibody	NULL		bind	NULL				MECA-79-positive CD34.IgG	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cell_105_7_957_s_100	11439191	(C) Binding  of MECA-79 antibody to MECA-79-positive CD34.IgG coated  on plates was measured in the absence  and presence of synthetic oligosaccharides, shown at right, at  different concentrations	bind
12871	1	4464	6	NULL	NULL	0	NULL	MECA-79 antibody	NULL		bind	NULL				MECA-79-positive CD34.IgG	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_105_7_957_s_100	11439191	(C) Binding  of MECA-79 antibody to MECA-79-positive CD34.IgG coated  on plates was measured in the absence  and presence of synthetic oligosaccharides, shown at right, at  different concentrations	bind
11286	1	4465	5	NULL	NULL	0	NULL	NK cells	NULL		bind	NULL				annexin V-FITC	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_3_810_s_139	15240120	(C) Binding  of NK cells to annexin V-FITC and propidium iodide (PI).	bind
11287	2	4465	5	NULL	NULL	0	NULL	NK cells	NULL		bind	NULL				PI	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_3_810_s_139	15240120	(C) Binding  of NK cells to annexin V-FITC and propidium iodide (PI).	bind
11288	3	4465	5	NULL	NULL	0	NULL	PI	NULL		is	NULL				propidium iodide	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_3_810_s_139	15240120	(C) Binding  of NK cells to annexin V-FITC and propidium iodide (PI).	bind
10773	1	4465	6	NULL	NULL	NULL	NULL	NK cells	Cell		bind					annexin V-FITC	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_3_810_s_139	15240120	(C) Binding  of NK cells to annexin V-FITC and propidium iodide (PI).	bind
10774	2	4465	6	NULL	NULL	NULL	NULL	NK cells	Cell		bind					propidium iodide	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_3_810_s_139	15240120	(C) Binding  of NK cells to annexin V-FITC and propidium iodide (PI).	bind
10775	3	4465	6	NULL	NULL	NULL	NULL	PI	Chemical		is					propidium iodide	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_3_810_s_139	15240120	(C) Binding  of NK cells to annexin V-FITC and propidium iodide (PI).	bind
11290	1	4467	5	NULL	NULL	0	NULL	ERK2	NULL		bind	NULL				GST-Elk-1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_710_s_317	9447967	(C) Binding and phosphorylation of GST-Elk-1 fusion proteins by ERK2.	bind
11291	2	4467	5	NULL	NULL	0	NULL	ERK2	NULL		phosphorylate	NULL				GST-Elk-1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_710_s_317	9447967	(C) Binding and phosphorylation of GST-Elk-1 fusion proteins by ERK2.	bind
44556	3	4467	5	10	NULL	0	NULL	GST-Elk-1	NULL		is a type of	NULL				fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_2_710_s_317	9447967	(C) Binding and phosphorylation of GST-Elk-1 fusion proteins by ERK2.	bind
10776	1	4467	6	NULL	NULL	NULL	NULL	ERK2	GP		bind					GST-Elk-1 	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_710_s_317	9447967	(C) Binding and phosphorylation of GST-Elk-1 fusion proteins by ERK2.	bind
10777	2	4467	6	NULL	NULL	NULL	NULL	ERK2	GP		phosphorylates					GST-Elk-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_710_s_317	9447967	(C) Binding and phosphorylation of GST-Elk-1 fusion proteins by ERK2.	bind
41477	3	4467	6	NULL	NULL	NULL	NULL	GST-Elk-1	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_710_s_317	9447967	(C) Binding and phosphorylation of GST-Elk-1 fusion proteins by ERK2.	bind
11292	1	4468	5	NULL	NULL	0	NULL	ER	NULL		bind	NULL				TIF2	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_312_3_656_s_63	14680815	(C) Binding between ER  and TIF2 was examined using the mammalian two-hybrid  system.	bind
10778	1	4468	6	NULL	NULL	NULL	NULL	ER	GP		bind					TIF2	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_312_3_656_s_63	14680815	(C) Binding between ER  and TIF2 was examined using the mammalian two-hybrid  system.	bind
11293	1	4469	5	10	NULL	0	NULL	IL-8	NULL		bind	NULL				CXCR1-CFP receptors	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5752_s_80	15964828	(c) Binding curve of IL-8 with CXCR1-CFP receptors  expressed in CX1-HEK cells.	bind
44558	2	4469	5	10	NULL	0	NULL	 CXCR1-CFP receptors	NULL		expressed in	NULL				CX1-HEK cells	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5752_s_80	15964828	(c) Binding curve of IL-8 with CXCR1-CFP receptors  expressed in CX1-HEK cells.	bind
10779	1	4469	6	NULL	NULL	NULL	NULL	IL-8	GP		bind					CXCR1-CFP receptors	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5752_s_80	15964828	(c) Binding curve of IL-8 with CXCR1-CFP receptors  expressed in CX1-HEK cells.	bind
41478	2	4469	6	NULL	NULL	NULL	NULL	CXCR1-CFP receptors	GP		are expressed in					CX1-HEK cells 	Cell				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5752_s_80	15964828	(c) Binding curve of IL-8 with CXCR1-CFP receptors  expressed in CX1-HEK cells.	bind
11294	1	4470	5	10	NULL	0	NULL	MDMX			bind					p53					NULL	H1299 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_15_6509_s_157	16024788	(c) Binding efficiency between  MDMX and p53 was determined by transient cotransfection of H1299 cells with MDMX  and p53 expression plasmids, followed by MDMX IP/p53 Western blotting.	bind
10780	1	4470	6	NULL	NULL	NULL	NULL	MDMX	GP		bind					p53	GP				NULL	H1299 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_15_6509_s_157	16024788	(c) Binding efficiency between  MDMX and p53 was determined by transient cotransfection of H1299 cells with MDMX  and p53 expression plasmids, followed by MDMX IP/p53 Western blotting.	bind
11295	1	4472	5	NULL	NULL	0	NULL	Sox-2	NULL		bind	NULL				UTF1	NULL			regulatory element	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_8_5453_s_179	10409735	(C) Binding modes of Sox-2 and Oct-3/4 to the UTF1 regulatory element.	bind
11296	2	4472	5	NULL	NULL	0	NULL	Oct-3/4	NULL		bind	NULL				UTF1	NULL			regulatory element	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_8_5453_s_179	10409735	(C) Binding modes of Sox-2 and Oct-3/4 to the UTF1 regulatory element.	bind
10781	1	4472	6	NULL	NULL	NULL	NULL	Sox-2	GP		bind					UTF-1	GP			regulatory element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5453_s_179	10409735	(C) Binding modes of Sox-2 and Oct-3/4 to the UTF1 regulatory element.	bind
10782	2	4472	6	NULL	NULL	NULL	NULL	Oct-3/4	GP		bind					UTF-1	GP			regulatory element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5453_s_179	10409735	(C) Binding modes of Sox-2 and Oct-3/4 to the UTF1 regulatory element.	bind
11297	1	4473	5	NULL	NULL	0	NULL	 calmodulin	NULL		bind	NULL				L-selectin	NULL		cytoplasmic tail		NULL		0	NULL	NULL	NULL	gw60_cell_92_6_809_s_108	9529256	(C) Binding of  calmodulin to the L-selectin cytoplasmic tail is inhibited by trifluoperazine.	bind
11298	2	4473	5	NULL	NULL	0	NULL	trifluoperazine	NULL		inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_92_6_809_s_108	9529256	(C) Binding of  calmodulin to the L-selectin cytoplasmic tail is inhibited by trifluoperazine.	bind
10783	1	4473	6	NULL	NULL	NULL	NULL	calmodulin	GP		bind					L-selectin	GP		cytoplasmic tail		NULL		NULL	NULL	NULL	NULL	gw60_cell_92_6_809_s_108	9529256	(C) Binding of  calmodulin to the L-selectin cytoplasmic tail is inhibited by trifluoperazine.	bind
10784	2	4473	6	NULL	NULL	NULL	NULL	trifluoperazine	Chemical		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_92_6_809_s_108	9529256	(C) Binding of  calmodulin to the L-selectin cytoplasmic tail is inhibited by trifluoperazine.	bind
11300	2	4474	5	NULL	NULL	0	NULL	4.1R/GST	NULL		bind	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_1_29_s_225	10189366	(C) Binding of 4.1R/GST to NuMA amino acid  sequence 1697-1889 translated from NuMA2/TOPO.	bind
11302	1	4474	5	NULL	NULL	0	NULL	NuMA	NULL		translated from	NULL		amino acid sequence 1697-1889		NuMA2/TOPO	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_1_29_s_225	10189366	(C) Binding of 4.1R/GST to NuMA amino acid  sequence 1697-1889 translated from NuMA2/TOPO.	bind
10785	1	4474	6	NULL	NULL	NULL	NULL	4.1R/GST	GP		bind					NuMA 	GP		amino acid sequence 1697-1889		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_1_29_s_225	10189366	(C) Binding of 4.1R/GST to NuMA amino acid  sequence 1697-1889 translated from NuMA2/TOPO.	bind
10786	2	4474	6	NULL	NULL	NULL	NULL	NuMA 	GP		translated from			amino acid sequence 1697-1889		NuMA2/TOPO	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_1_29_s_225	10189366	(C) Binding of 4.1R/GST to NuMA amino acid  sequence 1697-1889 translated from NuMA2/TOPO.	bind
11304	2	4475	5	10	NULL	0	NULL	4BP-1			bind					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_6041_s_135	10454551	(C) Binding of 4BP-1 to eIF-4E (bound to m7-GTP resin) was determined in the presence or absence of rapamycin (0.2 muM).	bind
54305	1	4475	5	10	NULL	0	NULL	 eIF-4E			bind					m7-GTP resin					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6041_s_135	10454551	(C) Binding of 4BP-1 to eIF-4E (bound to m7-GTP resin) was determined in the presence or absence of rapamycin (0.2 muM).	bind
10787	1	4475	6	NULL	NULL	NULL	NULL	eIF-4E	GP		bind					m7-GTP resin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_6041_s_135	10454551	(C) Binding of 4BP-1 to eIF-4E (bound to m7-GTP resin) was determined in the presence or absence of rapamycin (0.2 muM).	bind
10788	2	4475	6	NULL	NULL	NULL	NULL	4BP-1	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_6041_s_135	10454551	(C) Binding of 4BP-1 to eIF-4E (bound to m7-GTP resin) was determined in the presence or absence of rapamycin (0.2 muM).	bind
11306	1	4476	5	NULL	NULL	0	NULL	Abf2p	NULL		bind	NULL				four-way junction DNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1522_3_175_s_225	11779632	(C) Binding of Abf2p and phosphorylated Abf2p to four-way junction DNA.	bind
11308	2	4476	5	NULL	NULL	0	NULL	Abf2p	NULL	phosphorylated	bind	NULL				four-way junction DNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1522_3_175_s_225	11779632	(C) Binding of Abf2p and phosphorylated Abf2p to four-way junction DNA.	bind
10789	1	4476	6	NULL	NULL	NULL	NULL	Abf2p	GP		bind					four-way junction DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1522_3_175_s_225	11779632	(C) Binding of Abf2p and phosphorylated Abf2p to four-way junction DNA.	bind
10790	2	4476	6	NULL	NULL	NULL	NULL	Abf2p	GP	phosphorylated	bind					four-way junction DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1522_3_175_s_225	11779632	(C) Binding of Abf2p and phosphorylated Abf2p to four-way junction DNA.	bind
11309	1	4478	5	NULL	NULL	0	NULL	B-Myb	NULL		bind	NULL				NLK	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4705_s_137	16055500	(C) Binding of B-Myb to NLK  and HIPK2.	bind
11310	2	4478	5	NULL	NULL	0	NULL	B-Myb	NULL		bind	NULL				HIPK2	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4705_s_137	16055500	(C) Binding of B-Myb to NLK  and HIPK2.	bind
10791	1	4478	6	NULL	NULL	NULL	NULL	B-Myb	GP		bind					NLK	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4705_s_137	16055500	(C) Binding of B-Myb to NLK  and HIPK2.	bind
10792	2	4478	6	NULL	NULL	NULL	NULL	B-Myb	GP		bind					HIPK2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4705_s_137	16055500	(C) Binding of B-Myb to NLK  and HIPK2.	bind
11311	1	4479	5	NULL	NULL	0	NULL	Sir3p protein	NULL		bind	NULL				telomeric sequences	NULL				NULL	nocodazole-arrested (G2/M) phase cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4202_s_217	12024033	(C) Binding of both Sir3p and Dna2-Myc protein to telomeric sequences in nocodazole-arrested (G2/M) phase cells.	bind
11312	2	4479	5	NULL	NULL	0	NULL	Dna2-Myc protein	NULL		bind	NULL				telomeric sequences	NULL				NULL	nocodazole-arrested (G2/M) phase cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4202_s_217	12024033	(C) Binding of both Sir3p and Dna2-Myc protein to telomeric sequences in nocodazole-arrested (G2/M) phase cells.	bind
10793	1	4479	6	NULL	NULL	NULL	NULL	Sir3p	GP		bind					telomeric sequences					NULL	nocodazole-arrested (G2/M) phase cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4202_s_217	12024033	(C) Binding of both Sir3p and Dna2-Myc protein to telomeric sequences in nocodazole-arrested (G2/M) phase cells.	bind
10794	2	4479	6	NULL	NULL	NULL	NULL	Dna2-Myc protein	GP		bind					telomeric sequences					NULL	nocodazole-arrested (G2/M) phase cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4202_s_217	12024033	(C) Binding of both Sir3p and Dna2-Myc protein to telomeric sequences in nocodazole-arrested (G2/M) phase cells.	bind
11314	1	4480	5	NULL	NULL	0	NULL	CBP	NULL		bind	NULL				xUBF	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_6_5_1059_s_134	11106745	(C) Binding of CBP and Rb to xUBF are mutually exclusive.	bind
11315	2	4480	5	NULL	NULL	0	NULL	Rb	NULL		bind	NULL				xUBF	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_6_5_1059_s_134	11106745	(C) Binding of CBP and Rb to xUBF are mutually exclusive.	bind
11316	3	4480	5	NULL	NULL	0	NULL	statement 1	NULL		mutually exclusive to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_6_5_1059_s_134	11106745	(C) Binding of CBP and Rb to xUBF are mutually exclusive.	bind
10974	1	4480	6	NULL	NULL	NULL	NULL	CBP	GP		bind					xUBF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_5_1059_s_134	11106745	(C) Binding of CBP and Rb to xUBF are mutually exclusive.	bind
10975	2	4480	6	NULL	NULL	NULL	NULL	Rb	GP		bind					xUBF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_5_1059_s_134	11106745	(C) Binding of CBP and Rb to xUBF are mutually exclusive.	bind
10976	3	4480	6	NULL	NULL	NULL	NULL	statement 1	Process		is independent of					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_5_1059_s_134	11106745	(C) Binding of CBP and Rb to xUBF are mutually exclusive.	bind
11318	1	4481	5	NULL	NULL	0	NULL	Cdh1	NULL		bind	NULL				TPX2	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_23_10516_s_204	16287863	(C) Binding of Cdh1 to TPX2 and TPX2-N.	bind
11320	2	4481	5	10	NULL	0	NULL	Cdh1			bind					TPX2			N-terminus		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10516_s_204	16287863	(C) Binding of Cdh1 to TPX2 and TPX2-N.	bind
10977	1	4481	6	NULL	NULL	NULL	NULL	Cdh1	GP		bind					TPX2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10516_s_204	16287863	(C) Binding of Cdh1 to TPX2 and TPX2-N.	bind
10978	2	4481	6	NULL	NULL	NULL	NULL	Cdh1	GP		bind					TPX2	GP		N-terminus		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10516_s_204	16287863	(C) Binding of Cdh1 to TPX2 and TPX2-N.	bind
11323	1	4482	5	NULL	NULL	0	NULL	CMV gB	NULL		bind	NULL				DC-SIGNR	NULL				NULL		0	NULL	NULL	NULL	gw60_immunity_17_5_653_s_186	12433371	(C) Binding of CMV gB to DC-SIGNR.	bind
10979	1	4482	6	NULL	NULL	NULL	NULL	CMV gB	GP		bind					DC-SIGNR	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_5_653_s_186	12433371	(C) Binding of CMV gB to DC-SIGNR.	bind
11324	1	4483	5	10	NULL	0	NULL	collagen	NULL		bind	NULL				collagen substrates	NULL				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_5_2319_s_238	10225890	(C) Binding of collagen to different collagen substrates.	bind
10980	1	4483	6	NULL	NULL	NULL	NULL	collagen	GP		bind					collagen substrates	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_5_2319_s_238	10225890	(C) Binding of collagen to different collagen substrates.	bind
11326	1	4484	5	NULL	NULL	0	NULL	CPEB	NULL		bind	NULL				 XPum	NULL		Puf		NULL		0	NULL	NULL	NULL	gw70_mechdev_120_8_865_s_80	12963108	(C) Binding of CPEB to XPum Puf  but not to XPum NN and NC.	bind
11327	2	4484	5	NULL	NULL	0	NULL	CPEB	NULL		does not bind	NULL				XPum	NULL		NN		NULL		0	NULL	NULL	NULL	gw70_mechdev_120_8_865_s_80	12963108	(C) Binding of CPEB to XPum Puf  but not to XPum NN and NC.	bind
11328	3	4484	5	10	NULL	0	NULL	CPEB			does not bind					XPum			NC		NULL		NULL	NULL	NULL	NULL	gw70_mechdev_120_8_865_s_80	12963108	(C) Binding of CPEB to XPum Puf  but not to XPum NN and NC.	bind
10981	1	4484	6	NULL	NULL	NULL	NULL	CPEB	GP		bind					XPum	GP		puf		NULL		NULL	NULL	NULL	NULL	gw70_mechdev_120_8_865_s_80	12963108	(C) Binding of CPEB to XPum Puf  but not to XPum NN and NC.	bind
10982	2	4484	6	NULL	NULL	NULL	NULL	CPEB	GP		does not bind					XPum	GP		NN		NULL		NULL	NULL	NULL	NULL	gw70_mechdev_120_8_865_s_80	12963108	(C) Binding of CPEB to XPum Puf  but not to XPum NN and NC.	bind
10983	3	4484	6	NULL	NULL	NULL	NULL	CPEB	GP		does not bind					XPum	GP		NC		NULL		NULL	NULL	NULL	NULL	gw70_mechdev_120_8_865_s_80	12963108	(C) Binding of CPEB to XPum Puf  but not to XPum NN and NC.	bind
11337	1	4485	5	NULL	NULL	0	NULL	CtBP1	NULL		bind	NULL				deltaEF1	NULL	full-length			NULL	in vitro	0	NULL	NULL	NULL	gw60_molcellbiol_19_12_8581_s_125	10567582	(C) Binding of CtBP1 and CtBP2 to full-length deltaEF1 in vitro.	bind
11338	2	4485	5	NULL	NULL	0	NULL	CtBP2	NULL		bind	NULL				deltaEF1	NULL	full-length			NULL	in vitro	0	NULL	NULL	NULL	gw60_molcellbiol_19_12_8581_s_125	10567582	(C) Binding of CtBP1 and CtBP2 to full-length deltaEF1 in vitro.	bind
10984	1	4485	6	NULL	NULL	NULL	NULL	CtBP1	GP		bind					deltaEF1	GP	full length			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8581_s_125	10567582	(C) Binding of CtBP1 and CtBP2 to full-length deltaEF1 in vitro.	bind
10985	2	4485	6	NULL	NULL	NULL	NULL	CtBP2	GP		bind					deltaEF1	GP	full length			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8581_s_125	10567582	(C) Binding of CtBP1 and CtBP2 to full-length deltaEF1 in vitro.	bind
11339	1	4486	5	NULL	NULL	0	NULL	CtBP1	NULL		bind	NULL		K428R		Smad6	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_11_5_1389_s_122	12769861	(C) Binding of CtBP1(K428R) to Smad6 remains unchanged.	bind
10987	1	4486	6	NULL	NULL	NULL	NULL	CtBP1	GP		bind			K428R		Smad6	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_5_1389_s_122	12769861	(C) Binding of CtBP1(K428R) to Smad6 remains unchanged.	bind
11340	1	4487	5	NULL	NULL	0	NULL	DNA replication proteins	NULL		bind	NULL				chromatin	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_11_2_329_s_222	12620222	(C) Binding of DNA replication proteins and other checkpoint proteins to chromatin in the absence of Claspin.	bind
11341	2	4487	5	NULL	NULL	0	NULL	statement 1	NULL		in the absence of	NULL				Claspin	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_11_2_329_s_222	12620222	(C) Binding of DNA replication proteins and other checkpoint proteins to chromatin in the absence of Claspin.	bind
11342	3	4487	5	10	NULL	0	NULL	checkpoint proteins			bind					chromatin					NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_2_329_s_222	12620222	(C) Binding of DNA replication proteins and other checkpoint proteins to chromatin in the absence of Claspin.	bind
11343	4	4487	5	NULL	NULL	0	NULL	statement 3	NULL		in the absence of	NULL				Claspin	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_11_2_329_s_222	12620222	(C) Binding of DNA replication proteins and other checkpoint proteins to chromatin in the absence of Claspin.	bind
10988	1	4487	6	NULL	NULL	NULL	NULL	DNA replication proteins	GP		bind					chromatin	Chromosome				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_2_329_s_222	12620222	(C) Binding of DNA replication proteins and other checkpoint proteins to chromatin in the absence of Claspin.	bind
10989	2	4487	6	NULL	NULL	NULL	NULL	checkpoint proteins	GP		bind					chromatin	Chromosome				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_2_329_s_222	12620222	(C) Binding of DNA replication proteins and other checkpoint proteins to chromatin in the absence of Claspin.	bind
10990	3	4487	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs in absence of					Claspin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_2_329_s_222	12620222	(C) Binding of DNA replication proteins and other checkpoint proteins to chromatin in the absence of Claspin.	bind
10992	4	4487	6	NULL	NULL	NULL	NULL	statement 2	Process		occurs in absence of					Claspin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_2_329_s_222	12620222	(C) Binding of DNA replication proteins and other checkpoint proteins to chromatin in the absence of Claspin.	bind
11344	1	4488	5	NULL	NULL	0	NULL	DpiA protein	NULL		bind	NULL				pSC101 origin fragment	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_20_6025_s_75	14526013	(C) Binding of DpiA protein and the mutant proteins to pSC101 origin fragment.	bind
11345	2	4488	5	NULL	NULL	0	NULL	DpiA protein	NULL	mutant	bind	NULL				pSC101 origin fragment	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_20_6025_s_75	14526013	(C) Binding of DpiA protein and the mutant proteins to pSC101 origin fragment.	bind
10993	1	4488	6	NULL	NULL	NULL	NULL	DpiA protein	GP		bind					pSC101 origin fragment	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_20_6025_s_75	14526013	(C) Binding of DpiA protein and the mutant proteins to pSC101 origin fragment.	bind
10996	2	4488	6	NULL	NULL	NULL	NULL	DpiA protein	GP	mutant	bind					pSC101 origin fragment	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_20_6025_s_75	14526013	(C) Binding of DpiA protein and the mutant proteins to pSC101 origin fragment.	bind
11346	1	4489	5	10	NULL	0	NULL	E2F1			bind					MCM4					NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_10_4546_s_99	15121871	(C) Binding of E2F1 to E2F targets ( MCM4,  MCM3,  PCNA, and  p107) and control promoter ( AchR).	bind
11347	2	4489	5	10	NULL	0	NULL	E2F1			bind					MCM3					NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_10_4546_s_99	15121871	(C) Binding of E2F1 to E2F targets ( MCM4,  MCM3,  PCNA, and  p107) and control promoter ( AchR).	bind
11348	3	4489	5	10	NULL	0	NULL	E2F1			bind					PCNA					NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_10_4546_s_99	15121871	(C) Binding of E2F1 to E2F targets ( MCM4,  MCM3,  PCNA, and  p107) and control promoter ( AchR).	bind
11349	4	4489	5	10	NULL	0	NULL	E2F1			bind					 p107					NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_10_4546_s_99	15121871	(C) Binding of E2F1 to E2F targets ( MCM4,  MCM3,  PCNA, and  p107) and control promoter ( AchR).	bind
11350	5	4489	5	NULL	NULL	0	NULL	E2F1	NULL		bind	NULL				AchR	NULL	control		promoter	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_10_4546_s_99	15121871	(C) Binding of E2F1 to E2F targets ( MCM4,  MCM3,  PCNA, and  p107) and control promoter ( AchR).	bind
54364	6	4489	5	10	NULL	0	NULL	MCM4			is a type of					E2F target					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_10_4546_s_99	15121871	(C) Binding of E2F1 to E2F targets ( MCM4,  MCM3,  PCNA, and  p107) and control promoter ( AchR).	bind
54365	7	4489	5	10	NULL	0	NULL	MCM3			is a type of					E2F target					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_10_4546_s_99	15121871	(C) Binding of E2F1 to E2F targets ( MCM4,  MCM3,  PCNA, and  p107) and control promoter ( AchR).	bind
54366	8	4489	5	10	NULL	0	NULL	PCNA			is a type of					E2F target					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_10_4546_s_99	15121871	(C) Binding of E2F1 to E2F targets ( MCM4,  MCM3,  PCNA, and  p107) and control promoter ( AchR).	bind
54367	9	4489	5	10	NULL	0	NULL	p107			is a type of					E2F target					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_10_4546_s_99	15121871	(C) Binding of E2F1 to E2F targets ( MCM4,  MCM3,  PCNA, and  p107) and control promoter ( AchR).	bind
10997	1	4489	6	NULL	NULL	NULL	NULL	E2F1	GP		bind					MCM4	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_10_4546_s_99	15121871	(C) Binding of E2F1 to E2F targets ( MCM4,  MCM3,  PCNA, and  p107) and control promoter ( AchR).	bind
10998	2	4489	6	NULL	NULL	NULL	NULL	E2F1	GP		bind					MCM3	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_10_4546_s_99	15121871	(C) Binding of E2F1 to E2F targets ( MCM4,  MCM3,  PCNA, and  p107) and control promoter ( AchR).	bind
10999	3	4489	6	NULL	NULL	NULL	NULL	E2F1	GP		bind					PCNA	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_10_4546_s_99	15121871	(C) Binding of E2F1 to E2F targets ( MCM4,  MCM3,  PCNA, and  p107) and control promoter ( AchR).	bind
11000	4	4489	6	NULL	NULL	NULL	NULL	E2F1	GP		bind					p107	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_10_4546_s_99	15121871	(C) Binding of E2F1 to E2F targets ( MCM4,  MCM3,  PCNA, and  p107) and control promoter ( AchR).	bind
11002	5	4489	6	NULL	NULL	NULL	NULL	E2F1	GP		bind					AchR	GP	control		promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_10_4546_s_99	15121871	(C) Binding of E2F1 to E2F targets ( MCM4,  MCM3,  PCNA, and  p107) and control promoter ( AchR).	bind
54368	6	4489	6	NULL	NULL	NULL	NULL	MCM4	GP		is a type of					E2F target	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_10_4546_s_99	15121871	(C) Binding of E2F1 to E2F targets ( MCM4,  MCM3,  PCNA, and  p107) and control promoter ( AchR).	bind
54369	7	4489	6	NULL	NULL	NULL	NULL	MCM3	GP		is a type of					E2F target	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_10_4546_s_99	15121871	(C) Binding of E2F1 to E2F targets ( MCM4,  MCM3,  PCNA, and  p107) and control promoter ( AchR).	bind
54370	8	4489	6	NULL	NULL	NULL	NULL	PCNA	GP		is a type of					E2F target	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_10_4546_s_99	15121871	(C) Binding of E2F1 to E2F targets ( MCM4,  MCM3,  PCNA, and  p107) and control promoter ( AchR).	bind
54371	9	4489	6	NULL	NULL	NULL	NULL	p107	GP		is a type of					E2F target	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_10_4546_s_99	15121871	(C) Binding of E2F1 to E2F targets ( MCM4,  MCM3,  PCNA, and  p107) and control promoter ( AchR).	bind
11351	1	4490	5	NULL	NULL	0	NULL	EL229C-B	NULL		bind	NULL				GroES	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_107_2_223_s_78	11672529	(C) Binding of EL229C-B and  EL229C-B:SA complex to GroES analyzed by surface  plasmon resonance in the presence of ATP.	bind
11352	2	4490	5	NULL	NULL	0	NULL	statement 1	NULL		in the presence of	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_107_2_223_s_78	11672529	(C) Binding of EL229C-B and  EL229C-B:SA complex to GroES analyzed by surface  plasmon resonance in the presence of ATP.	bind
11353	3	4490	5	NULL	NULL	0	NULL	EL229C-B:SA complex	NULL		bind	NULL				GroES	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_107_2_223_s_78	11672529	(C) Binding of EL229C-B and  EL229C-B:SA complex to GroES analyzed by surface  plasmon resonance in the presence of ATP.	bind
11354	4	4490	5	NULL	NULL	0	NULL	statement 3	NULL		in the presence of	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_107_2_223_s_78	11672529	(C) Binding of EL229C-B and  EL229C-B:SA complex to GroES analyzed by surface  plasmon resonance in the presence of ATP.	bind
11003	1	4490	6	NULL	NULL	NULL	NULL	EL229C-B	GP		bind					GroES	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_78	11672529	(C) Binding of EL229C-B and  EL229C-B:SA complex to GroES analyzed by surface  plasmon resonance in the presence of ATP.	bind
11004	2	4490	6	NULL	NULL	NULL	NULL	EL229C-B:SA complex	GP		bind					GroES	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_78	11672529	(C) Binding of EL229C-B and  EL229C-B:SA complex to GroES analyzed by surface  plasmon resonance in the presence of ATP.	bind
12872	3	4490	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs in presence of					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_78	11672529	(C) Binding of EL229C-B and  EL229C-B:SA complex to GroES analyzed by surface  plasmon resonance in the presence of ATP.	bind
12873	4	4490	6	NULL	NULL	NULL	NULL	statement 2	Process		occurs in presence of					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_78	11672529	(C) Binding of EL229C-B and  EL229C-B:SA complex to GroES analyzed by surface  plasmon resonance in the presence of ATP.	bind
11355	1	4491	5	NULL	NULL	0	NULL	fibronectin	NULL		bind	NULL				UspA2	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_9_4374_s_280	9712790	(C) Binding of fibronectin to UspA2.	bind
11018	1	4491	6	NULL	NULL	NULL	NULL	fibronectin	GP		bind					UspA2	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_9_4374_s_280	9712790	(C) Binding of fibronectin to UspA2.	bind
11356	1	4493	5	NULL	NULL	0	NULL	S2R+ cells	NULL		transfected with	NULL				Frizzled2-FLAG	NULL				NULL		0	NULL	NULL	NULL	gw70_development_132_24_5479_s_176	16291792	(C) Binding of GFP-Wingless to S2R+ cells transfected  with Frizzled2-FLAG.	bind
11357	2	4493	5	NULL	NULL	0	NULL	GFP-Wingless	NULL		bind	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_development_132_24_5479_s_176	16291792	(C) Binding of GFP-Wingless to S2R+ cells transfected  with Frizzled2-FLAG.	bind
11023	1	4493	6	NULL	NULL	NULL	NULL	S2R+ cells	Cell		transfected with					Frizzled2	GP	FLAG tagged			NULL		NULL	NULL	NULL	NULL	gw70_development_132_24_5479_s_176	16291792	(C) Binding of GFP-Wingless to S2R+ cells transfected  with Frizzled2-FLAG.	bind
11024	2	4493	6	NULL	NULL	NULL	NULL	GFP-wingless	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_132_24_5479_s_176	16291792	(C) Binding of GFP-Wingless to S2R+ cells transfected  with Frizzled2-FLAG.	bind
11358	1	4494	5	NULL	NULL	0	NULL	GLD-1	NULL		bind	NULL				mes-3	NULL			3' UTR	NULL		0	NULL	NULL	NULL	gw60_genetics_159_3_1007_s_196	11729149	(C) Binding of GLD-1 to the  mes-3 3' UTR was tested using RNA gel mobility shift assay.	bind
11026	1	4494	6	NULL	NULL	NULL	NULL	GLD-1	GP		bind					mes-3 	GP			3' UTR	NULL		NULL	NULL	NULL	NULL	gw60_genetics_159_3_1007_s_196	11729149	(C) Binding of GLD-1 to the  mes-3 3' UTR was tested using RNA gel mobility shift assay.	bind
11359	1	4495	5	NULL	NULL	0	NULL	GST-MBD2a	NULL		bind	NULL				RHA	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_molcellbiol_23_8_2645_s_164	12665568	(C) Binding of GST-MBD2a to RHA in vitro.	bind
11027	1	4495	6	NULL	NULL	NULL	NULL	GST-MBD2a	GP		bind					RHA	Chemical				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_23_8_2645_s_164	12665568	(C) Binding of GST-MBD2a to RHA in vitro.	bind
11360	1	4496	5	NULL	NULL	0	NULL	GST-VCA	NULL		bind	NULL				Arp2/3	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_150_6_1299_s_76	10995436	(C) Binding of GST-VCA (0.2 muM) to Arp2/3 (0.1 muM) was tested (as in B) in the presence of the indicated concentrations of HT-WG or HT-WGP.	bind
11361	2	4496	5	NULL	NULL	0	NULL	statement 1	NULL		in the presence of	NULL				HT-WG	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_150_6_1299_s_76	10995436	(C) Binding of GST-VCA (0.2 muM) to Arp2/3 (0.1 muM) was tested (as in B) in the presence of the indicated concentrations of HT-WG or HT-WGP.	bind
11362	3	4496	5	NULL	NULL	0	NULL	statement 1	NULL		in the presence of	NULL				HT-WGP	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_150_6_1299_s_76	10995436	(C) Binding of GST-VCA (0.2 muM) to Arp2/3 (0.1 muM) was tested (as in B) in the presence of the indicated concentrations of HT-WG or HT-WGP.	bind
11363	4	4496	5	NULL	NULL	0	NULL	statement 2	NULL		is an alternative to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_150_6_1299_s_76	10995436	(C) Binding of GST-VCA (0.2 muM) to Arp2/3 (0.1 muM) was tested (as in B) in the presence of the indicated concentrations of HT-WG or HT-WGP.	bind
11030	1	4496	6	NULL	NULL	NULL	NULL	GST-VCA	GP		bind					Arp2/3	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_150_6_1299_s_76	10995436	(C) Binding of GST-VCA (0.2 muM) to Arp2/3 (0.1 muM) was tested (as in B) in the presence of the indicated concentrations of HT-WG or HT-WGP.	bind
12874	2	4496	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs in presence of					HT-WG	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_150_6_1299_s_76	10995436	(C) Binding of GST-VCA (0.2 muM) to Arp2/3 (0.1 muM) was tested (as in B) in the presence of the indicated concentrations of HT-WG or HT-WGP.	bind
12875	3	4496	6	NULL	NULL	NULL	NULL	statement 2	Process		occurs in presence of					HT-WGP	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_150_6_1299_s_76	10995436	(C) Binding of GST-VCA (0.2 muM) to Arp2/3 (0.1 muM) was tested (as in B) in the presence of the indicated concentrations of HT-WG or HT-WGP.	bind
12876	4	4496	6	NULL	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_150_6_1299_s_76	10995436	(C) Binding of GST-VCA (0.2 muM) to Arp2/3 (0.1 muM) was tested (as in B) in the presence of the indicated concentrations of HT-WG or HT-WGP.	bind
11364	1	4497	5	10	NULL	0	NULL	Ikaros		immunopurified	bind					mononucleosomes 					NULL		NULL	NULL	NULL	NULL	gw60_immunity_10_3_345_s_141	10204490	(C) Binding of immunopurified Ikaros to mononucleosomes (Nc).	bind
11031	1	4497	6	NULL	NULL	NULL	NULL	Ikaros	GP	immunopurified	bind					mononucleosomes	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_10_3_345_s_141	10204490	(C) Binding of immunopurified Ikaros to mononucleosomes (Nc).	bind
11365	1	4498	5	NULL	NULL	0	NULL	Mad2	NULL		bind	NULL				Cdc20 fragments	NULL				NULL	in wild-type cells	0	NULL	NULL	NULL	gw60_molcell_12_1_87_s_251	12887895	(C) Binding of Mad2 to Cdc20 fragments in wild-type and  cct1-2 cells.	bind
11366	2	4498	5	NULL	NULL	0	NULL	Mad2	NULL		bind	NULL				Cdc20 fragments	NULL				NULL	in cct1-2 cells	0	NULL	NULL	NULL	gw60_molcell_12_1_87_s_251	12887895	(C) Binding of Mad2 to Cdc20 fragments in wild-type and  cct1-2 cells.	bind
11032	1	4498	6	NULL	NULL	NULL	NULL	Mad2	GP		bind					Cdc20 fragment	AminoAcid				NULL	wild-type cells	NULL	NULL	NULL	NULL	gw60_molcell_12_1_87_s_251	12887895	(C) Binding of Mad2 to Cdc20 fragments in wild-type and  cct1-2 cells.	bind
12877	2	4498	6	NULL	NULL	NULL	NULL	Mad2	GP		bind					Cdc20 fragment	AminoAcid				NULL	cct1-2 cells	NULL	NULL	NULL	NULL	gw60_molcell_12_1_87_s_251	12887895	(C) Binding of Mad2 to Cdc20 fragments in wild-type and  cct1-2 cells.	bind
11367	1	4499	5	NULL	NULL	0	NULL	mPER	NULL		bind	NULL				CKI	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_2_584_s_246	14701732	(C) Binding of mPER with CKI .	bind
11033	1	4499	6	NULL	NULL	NULL	NULL	mPER	GP		bind					CKI	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_2_584_s_246	14701732	(C) Binding of mPER with CKI .	bind
11368	1	4500	5	10	NULL	0	NULL	mSin3A-HDAC-1	NULL		bind	NULL					NULL		ETS domains		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_8_2802_s_140	11283259	(C) Binding of mSin3A-HDAC-1 to different ETS domains.	bind
11034	1	4500	6	NULL	NULL	NULL	NULL	mSin3A-HDAC-1	GP		bind								ETS domain		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_8_2802_s_140	11283259	(C) Binding of mSin3A-HDAC-1 to different ETS domains.	bind
11369	1	4501	5	NULL	NULL	0	NULL	n-sec1	NULL		bind	NULL				syntaxin 1a	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_16_6_1229_s_90	8663999	(C) Binding of n-sec1 to syntaxin 1a in the presence of 1 mM S-NC.	bind
11370	2	4501	5	NULL	NULL	0	NULL	statement 1	NULL		in the presence of	NULL				S-NC	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_16_6_1229_s_90	8663999	(C) Binding of n-sec1 to syntaxin 1a in the presence of 1 mM S-NC.	bind
11035	1	4501	6	NULL	NULL	NULL	NULL	n-sec1	GP		bind					syntaxin 1a	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_16_6_1229_s_90	8663999	(C) Binding of n-sec1 to syntaxin 1a in the presence of 1 mM S-NC.	bind
11036	2	4501	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs in presence of					S-NC	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_16_6_1229_s_90	8663999	(C) Binding of n-sec1 to syntaxin 1a in the presence of 1 mM S-NC.	bind
11371	1	4502	5	NULL	NULL	0	NULL	nuclear proteins	NULL		bind	NULL				TGF- 1	NULL	human		AP-1 site B of promoter	NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_304_2_301_s_95	12711314	(C) Binding of nuclear proteins to the AP-1 site B of the human TGF- 1 promoter.	bind
11037	1	4502	6	NULL	NULL	NULL	NULL	nuclear proteins	GP		bind					TGF-1	GP	human		AP-1 site B of promoter	NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_304_2_301_s_95	12711314	(C) Binding of nuclear proteins to the AP-1 site B of the human TGF- 1 promoter.	bind
11372	1	4503	5	NULL	NULL	0	NULL	Nup98	NULL		bind	NULL				VSV M protein	NULL				NULL		0	NULL	NULL	NULL	gw70_microbesinfect_6_8_715_s_170	15207818	(C) Binding of Nup98 to VSV M protein.	bind
11044	1	4503	6	NULL	NULL	NULL	NULL	Nup98	GP		bind					VSV M protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbesinfect_6_8_715_s_170	15207818	(C) Binding of Nup98 to VSV M protein.	bind
11373	1	4504	5	NULL	NULL	0	NULL	p107	NULL		bind	NULL				cyclin - Cdk2 complexes	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_168_1_55_s_72	15631990	(C) Binding of p107 to cyclin - Cdk2 complexes.	bind
11046	1	4504	6	NULL	NULL	NULL	NULL	p107	GP		bind					cyclin - Cdk2 complexes	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_1_55_s_72	15631990	(C) Binding of p107 to cyclin - Cdk2 complexes.	bind
11374	1	4505	5	NULL	NULL	0	NULL	p202	NULL		bind	NULL				MyoD protein	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_2_1074_s_258	9448005	(C) Binding of p202 to MyoD protein as assayed by coimmunoprecipitation.	bind
11047	1	4505	6	NULL	NULL	NULL	NULL	p202	GP		bind					MyoD	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_1074_s_258	9448005	(C) Binding of p202 to MyoD protein as assayed by coimmunoprecipitation.	bind
11375	1	4506	5	NULL	NULL	0	NULL	p53/p73	NULL		bind	NULL		DBD		MDM2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_24_8533_s_193	11713288	(C) Binding of p53/p73DBD or p53/p73betaeCT to MDM2 was examined as described for Fig.  3.	bind
11376	2	4506	5	NULL	NULL	0	NULL	p53/p73beta	NULL		bind	NULL		eCT		MDM2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_24_8533_s_193	11713288	(C) Binding of p53/p73DBD or p53/p73betaeCT to MDM2 was examined as described for Fig.  3.	bind
54372	3	4506	5	10	NULL	0	NULL	statement 1			is an alternative to					statement 2					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_24_8533_s_193	11713288	(C) Binding of p53/p73DBD or p53/p73betaeCT to MDM2 was examined as described for Fig.  3.	bind
11050	1	4506	6	NULL	NULL	NULL	NULL	p53/p73	GP		bind			DBD		MDM2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_24_8533_s_193	11713288	(C) Binding of p53/p73DBD or p53/p73betaeCT to MDM2 was examined as described for Fig.  3.	bind
11051	2	4506	6	NULL	NULL	NULL	NULL	p53/p73beta	GP		bind			eCT		MDM2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_24_8533_s_193	11713288	(C) Binding of p53/p73DBD or p53/p73betaeCT to MDM2 was examined as described for Fig.  3.	bind
11052	3	4506	6	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_24_8533_s_193	11713288	(C) Binding of p53/p73DBD or p53/p73betaeCT to MDM2 was examined as described for Fig.  3.	bind
11377	1	4507	5	NULL	NULL	0	NULL	p73beta/p53	NULL		bind	NULL		CT		MDM2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_24_8533_s_162	11713288	(C) Binding of p73beta/p53CT to MDM2 was analyzed by incubating lysates from cells expressing Flag-p73beta/p53CT with GST-MDM2.	bind
11057	1	4507	6	NULL	NULL	NULL	NULL	p73beta/p53	GP		bind			CT		MDM2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_24_8533_s_162	11713288	(C) Binding of p73beta/p53CT to MDM2 was analyzed by incubating lysates from cells expressing Flag-p73beta/p53CT with GST-MDM2.	bind
11378	1	4508	5	NULL	NULL	0	NULL	PAI-2	NULL		bind	NULL				Rb	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_18_6520_s_152	12944478	(C) Binding of PAI-2 and the C-D interhelical deletion mutant of PAI-2 to Rb and Rb LXCXE mutants.	bind
11379	2	4508	5	NULL	NULL	0	NULL	PAI-2	NULL		bind	NULL				Rb	NULL	mutant	LXCXE		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_18_6520_s_152	12944478	(C) Binding of PAI-2 and the C-D interhelical deletion mutant of PAI-2 to Rb and Rb LXCXE mutants.	bind
11380	3	4508	5	NULL	NULL	0	NULL	PAI-2	NULL	deletion mutants of	bind	NULL		C-D interhelical		Rb	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_18_6520_s_152	12944478	(C) Binding of PAI-2 and the C-D interhelical deletion mutant of PAI-2 to Rb and Rb LXCXE mutants.	bind
11381	4	4508	5	NULL	NULL	0	NULL	PAI-2	NULL	deletion mutants of	bind	NULL		C-D interhelical		Rb	NULL	mutant	LXCXE		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_18_6520_s_152	12944478	(C) Binding of PAI-2 and the C-D interhelical deletion mutant of PAI-2 to Rb and Rb LXCXE mutants.	bind
11060	1	4508	6	NULL	NULL	NULL	NULL	PAI-2	GP		bind					Rb	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6520_s_152	12944478	(C) Binding of PAI-2 and the C-D interhelical deletion mutant of PAI-2 to Rb and Rb LXCXE mutants.	bind
11061	2	4508	6	NULL	NULL	NULL	NULL	PAI-2	GP	deletion mutant	bind			C-D interhelical		Rb	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6520_s_152	12944478	(C) Binding of PAI-2 and the C-D interhelical deletion mutant of PAI-2 to Rb and Rb LXCXE mutants.	bind
11062	3	4508	6	NULL	NULL	NULL	NULL	PAI-2	GP		bind					Rb	GP	mutant	LXCXE		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6520_s_152	12944478	(C) Binding of PAI-2 and the C-D interhelical deletion mutant of PAI-2 to Rb and Rb LXCXE mutants.	bind
11064	4	4508	6	NULL	NULL	NULL	NULL	PAI-2	GP	deletion mutant	bind			C-D interhelical		Rb	GP	mutant	LXCXE		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6520_s_152	12944478	(C) Binding of PAI-2 and the C-D interhelical deletion mutant of PAI-2 to Rb and Rb LXCXE mutants.	bind
11382	1	4509	5	NULL	NULL	0	NULL	PCNA	NULL		bind	NULL				CAF-1	NULL		p150 subunit		NULL		NULL	NULL	NULL	NULL	gw60_cell_96_4_575_s_144	10052459	(C) Binding of PCNA  to the p150 subunit of CAF-1.	bind
11066	1	4509	6	NULL	NULL	NULL	NULL	PCNA	GP		bind					CAF-1	GP		p150 subunit		NULL		NULL	NULL	NULL	NULL	gw60_cell_96_4_575_s_144	10052459	(C) Binding of PCNA  to the p150 subunit of CAF-1.	bind
11383	1	4510	5	NULL	NULL	0	NULL	sera	NULL	human;; pooled	bind	NULL				RESA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_9_4679_s_222	10456916	(C) Binding of pooled human sera to RESA and two synthetic mimotopes, 17(3) and 15(1).	bind
11384	2	4510	5	10	NULL	0	NULL	sera		human;; pooled	bind					mimotopes		synthetic			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_9_4679_s_222	10456916	(C) Binding of pooled human sera to RESA and two synthetic mimotopes, 17(3) and 15(1).	bind
11068	1	4510	6	NULL	NULL	NULL	NULL	sera	GP	pooled;; human	bind					RESA	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_9_4679_s_222	10456916	(C) Binding of pooled human sera to RESA and two synthetic mimotopes, 17(3) and 15(1).	bind
11070	2	4510	6	NULL	NULL	NULL	NULL	sera	GP	pooled;; human	bind					mimotopes	GP	synthetic			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_9_4679_s_222	10456916	(C) Binding of pooled human sera to RESA and two synthetic mimotopes, 17(3) and 15(1).	bind
11386	1	4511	5	NULL	NULL	0	NULL	p120 E4F protein	NULL	purified	bind	NULL				cyclin A	NULL			CRE site	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_8_2956_s_316	11283272	(C) Binding of purified p120 E4F protein to the cyclin A CRE site is enhanced by pRB.	bind
11387	2	4511	5	NULL	NULL	0	NULL	pRB	NULL		enhances	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_8_2956_s_316	11283272	(C) Binding of purified p120 E4F protein to the cyclin A CRE site is enhanced by pRB.	bind
11071	1	4511	6	NULL	NULL	NULL	NULL	p120 E4F protein	GP	purified	bind					cyclin A	GP			CRE site	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_8_2956_s_316	11283272	(C) Binding of purified p120 E4F protein to the cyclin A CRE site is enhanced by pRB.	bind
11072	2	4511	6	NULL	NULL	NULL	NULL	pRB	GP		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_8_2956_s_316	11283272	(C) Binding of purified p120 E4F protein to the cyclin A CRE site is enhanced by pRB.	bind
11388	1	4512	5	NULL	NULL	0	NULL	Rad9	NULL		bind	NULL				GST-BRCT	NULL				NULL	wild-type yeast extracts	0	NULL	NULL	NULL	gw60_currbiol_9_10_551_s_73	10339432	(c) Binding of Rad9 by GST-BRCT from wild-type yeast extracts.	bind
11076	1	4512	6	NULL	NULL	NULL	NULL	Rad9	GP		bind					GST-BRCT	GP				NULL	wild type yeast extracts	NULL	NULL	NULL	NULL	gw60_currbiol_9_10_551_s_73	10339432	(c) Binding of Rad9 by GST-BRCT from wild-type yeast extracts.	bind
11389	1	4513	5	NULL	NULL	0	NULL	E47	NULL	recombinant	bind	NULL				mb-1	NULL			promoter distal region	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_24_8539_s_241	12446773	(C) Binding of recombinant E47 to the  mb-1 promoter distal region.	bind
11091	1	4513	6	NULL	NULL	NULL	NULL	E47	GP	recombinant	bind					mb-1	GP			distal region of promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_24_8539_s_241	12446773	(C) Binding of recombinant E47 to the  mb-1 promoter distal region.	bind
11390	1	4514	5	NULL	NULL	0	NULL	GST-Myc	NULL	recombinant	bind	NULL				FasL	NULL			Myc-binding site in promoter	NULL		0	NULL	NULL	NULL	gw60_currbiol_10_19_1205_s_40	11050389	(c) Binding of recombinant GST-Myc and GST-Max to the Myc-binding site in the FasL promoter.	bind
11391	2	4514	5	NULL	NULL	0	NULL	GST-Max	NULL	recombinant	bind	NULL				FasL	NULL			Myc-binding site in promoter	NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_19_1205_s_40	11050389	(c) Binding of recombinant GST-Myc and GST-Max to the Myc-binding site in the FasL promoter.	bind
11097	1	4514	6	NULL	NULL	NULL	NULL	GST-Myc	GP	recombinant	bind					FasL	GP			Myc-binding site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_19_1205_s_40	11050389	(c) Binding of recombinant GST-Myc and GST-Max to the Myc-binding site in the FasL promoter.	bind
11098	2	4514	6	NULL	NULL	NULL	NULL	GST-Max	GP	recombinant	bind					FasL	GP			Myc-binding site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_19_1205_s_40	11050389	(c) Binding of recombinant GST-Myc and GST-Max to the Myc-binding site in the FasL promoter.	bind
11392	1	4515	5	NULL	NULL	0	NULL	RAS	NULL		activated by	NULL				EGF	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_3_916_s_144	11784866	(C) Binding of RIN1 to RAS activated by EGF.	bind
11393	2	4515	5	NULL	NULL	0	NULL	RIN1	NULL		bind	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_3_916_s_144	11784866	(C) Binding of RIN1 to RAS activated by EGF.	bind
11101	1	4515	6	NULL	NULL	NULL	NULL	EGF	GP		activates					RAS	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_3_916_s_144	11784866	(C) Binding of RIN1 to RAS activated by EGF.	bind
11103	2	4515	6	NULL	NULL	NULL	NULL	RIN1	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_3_916_s_144	11784866	(C) Binding of RIN1 to RAS activated by EGF.	bind
11394	1	4516	5	NULL	NULL	0	NULL	S-layer proteins	NULL		bind	NULL				type IV collagen	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_22_6440_s_237	11053389	(C) Binding of S-layer proteins to type IV and I collagens, laminin, fibronectin, and BSA immobilized on plastic.	bind
11395	2	4516	5	NULL	NULL	0	NULL	S-layer proteins	NULL		bind	NULL				type I collagen	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_22_6440_s_237	11053389	(C) Binding of S-layer proteins to type IV and I collagens, laminin, fibronectin, and BSA immobilized on plastic.	bind
11396	3	4516	5	NULL	NULL	0	NULL	S-layer proteins	NULL		bind	NULL				laminin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_22_6440_s_237	11053389	(C) Binding of S-layer proteins to type IV and I collagens, laminin, fibronectin, and BSA immobilized on plastic.	bind
11397	4	4516	5	NULL	NULL	0	NULL	S-layer proteins	NULL		bind	NULL				fibronectin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_22_6440_s_237	11053389	(C) Binding of S-layer proteins to type IV and I collagens, laminin, fibronectin, and BSA immobilized on plastic.	bind
11398	5	4516	5	10	NULL	0	NULL	S-layer proteins	NULL		bind	NULL				BSA	NULL	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_22_6440_s_237	11053389	(C) Binding of S-layer proteins to type IV and I collagens, laminin, fibronectin, and BSA immobilized on plastic.	bind
11105	1	4516	6	NULL	NULL	NULL	NULL	S-layer proteins	GP		bind					type IV collagen	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_22_6440_s_237	11053389	(C) Binding of S-layer proteins to type IV and I collagens, laminin, fibronectin, and BSA immobilized on plastic.	bind
11107	2	4516	6	NULL	NULL	NULL	NULL	S-layer proteins	GP		bind					type I collagen	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_22_6440_s_237	11053389	(C) Binding of S-layer proteins to type IV and I collagens, laminin, fibronectin, and BSA immobilized on plastic.	bind
11108	3	4516	6	NULL	NULL	NULL	NULL	S-layer proteins	GP		bind					laminin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_22_6440_s_237	11053389	(C) Binding of S-layer proteins to type IV and I collagens, laminin, fibronectin, and BSA immobilized on plastic.	bind
11109	4	4516	6	NULL	NULL	NULL	NULL	S-layer proteins	GP		bind					fibronectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_22_6440_s_237	11053389	(C) Binding of S-layer proteins to type IV and I collagens, laminin, fibronectin, and BSA immobilized on plastic.	bind
11110	5	4516	6	NULL	NULL	NULL	NULL	BSA	GP		immobilized on					plastic	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_22_6440_s_237	11053389	(C) Binding of S-layer proteins to type IV and I collagens, laminin, fibronectin, and BSA immobilized on plastic.	bind
11112	6	4516	6	NULL	NULL	NULL	NULL	S-layer proteins	GP		bind					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_22_6440_s_237	11053389	(C) Binding of S-layer proteins to type IV and I collagens, laminin, fibronectin, and BSA immobilized on plastic.	bind
11399	1	4517	5	NULL	NULL	0	NULL	NIH-3T3 cells	NULL		express	NULL				ErbB-2	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1525_1_191_s_124	11342269	(c) Binding of scFv-COS-1 cells to ErbB-2-expressing NIH-3T3 cells.	bind
11400	2	4517	5	NULL	NULL	0	NULL	scFv-COS-1 cells	NULL		bind	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1525_1_191_s_124	11342269	(c) Binding of scFv-COS-1 cells to ErbB-2-expressing NIH-3T3 cells.	bind
11114	1	4517	6	NULL	NULL	NULL	NULL	NIH-3T3 cells	Cell		express					ErbB-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1525_1_191_s_124	11342269	(c) Binding of scFv-COS-1 cells to ErbB-2-expressing NIH-3T3 cells.	bind
11116	2	4517	6	NULL	NULL	NULL	NULL	scFv-COS-1 cells	Cell		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1525_1_191_s_124	11342269	(c) Binding of scFv-COS-1 cells to ErbB-2-expressing NIH-3T3 cells.	bind
11401	1	4518	5	NULL	NULL	0	NULL	sperm cells	NULL		bind	NULL				ZP	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1469_3_197_s_830	11063883	(C) Binding of sperm cells to the ZP triggers the acrosome reaction and acrosomal enzymes are secreted.	bind
11402	2	4518	5	NULL	NULL	0	NULL	statement 1	NULL		triggers	NULL				acrosome	NULL	reaction of			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1469_3_197_s_830	11063883	(C) Binding of sperm cells to the ZP triggers the acrosome reaction and acrosomal enzymes are secreted.	bind
11403	3	4518	5	10	NULL	0	NULL	statement 2			leads to					acrosomal enzymes		secretion of			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1469_3_197_s_830	11063883	(C) Binding of sperm cells to the ZP triggers the acrosome reaction and acrosomal enzymes are secreted.	bind
11117	1	4518	6	NULL	NULL	NULL	NULL	sperm cells	Cell		bind					ZP	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1469_3_197_s_830	11063883	(C) Binding of sperm cells to the ZP triggers the acrosome reaction and acrosomal enzymes are secreted.	bind
11119	2	4518	6	NULL	NULL	NULL	NULL	statement 1	Process		triggers					acrosome	CellComponent	reaction of			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1469_3_197_s_830	11063883	(C) Binding of sperm cells to the ZP triggers the acrosome reaction and acrosomal enzymes are secreted.	bind
11122	3	4518	6	NULL	NULL	NULL	NULL	statement 2	Process		leads to 					acrosomal enzyme 	GP	secretion of			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1469_3_197_s_830	11063883	(C) Binding of sperm cells to the ZP triggers the acrosome reaction and acrosomal enzymes are secreted.	bind
11404	1	4519	5	NULL	NULL	0	NULL	JunB derivatives	NULL		bind	NULL				JNK2	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_87_5_929_s_128	8945519	(C) Binding of the different JunB  derivatives to JNK2.	bind
11123	1	4519	6	NULL	NULL	NULL	NULL	JunB derivatives	GP		bind					JNK2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_87_5_929_s_128	8945519	(C) Binding of the different JunB  derivatives to JNK2.	bind
11405	1	4520	5	NULL	NULL	0	NULL		NULL		bind	NULL		linker sequence		ERK2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_7_2_387_s_37	11239467	(C) Binding of the linker sequence to ERK2.	bind
11125	1	4520	6	NULL	NULL	NULL	NULL				bind			linker sequence		ERK2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_2_387_s_37	11239467	(C) Binding of the linker sequence to ERK2.	bind
11406	1	4521	5	NULL	NULL	0	NULL	M4	NULL	mutant	bind	NULL				nuclear matrix	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_7_4165_s_276	9632801	(C) Binding of the M4 and M5 mutants to the nuclear matrix.	bind
11407	2	4521	5	NULL	NULL	0	NULL	M5	NULL	mutant	bind	NULL				nuclear matrix	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_7_4165_s_276	9632801	(C) Binding of the M4 and M5 mutants to the nuclear matrix.	bind
11129	1	4521	6	NULL	NULL	NULL	NULL	M4		mutant	bind					nuclear matrix	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_4165_s_276	9632801	(C) Binding of the M4 and M5 mutants to the nuclear matrix.	bind
11131	2	4521	6	NULL	NULL	NULL	NULL	M5		mutant	bind					nuclear matrix	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_4165_s_276	9632801	(C) Binding of the M4 and M5 mutants to the nuclear matrix.	bind
11408	1	4522	5	10	NULL	0	NULL	THP-1 cells			bind					von Willebrand factor		deletion of	domain A2 		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_153_5_905_s_241	11381078	(C) Binding of THP-1 cells to domain A2 - deleted von Willebrand factor.	bind
11134	1	4522	6	NULL	NULL	NULL	NULL	THP-1 cells	Cell		bind					von Willebrand factor	GP	deletion of	domain A2		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_153_5_905_s_241	11381078	(C) Binding of THP-1 cells to domain A2 - deleted von Willebrand factor.	bind
11420	1	4523	5	10	NULL	0	NULL	vitronectin	NULL	 NHS	bind	NULL				H. influenzae strains	NULL	recombinant 			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_74_3_1597_s_270	16495531	(C) Binding of vitronectin from NHS by these recombinant  H. influenzae strains.	bind
11135	1	4523	6	NULL	NULL	NULL	NULL	H. influenzae strains	Organism	recombinant	bind					vitronectin	GP	NHS			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_74_3_1597_s_270	16495531	(C) Binding of vitronectin from NHS by these recombinant  H. influenzae strains.	bind
11409	1	4524	5	NULL	NULL	0	NULL	Vav-3	NULL	wild type	bind	NULL				RhoA	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_11_7870_s_274	10523675	(C) Binding of wild type Vav-3 to RhoA.	bind
11136	1	4524	6	NULL	NULL	NULL	NULL	Vav-3	GP	wild type	bind					RhoA	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_11_7870_s_274	10523675	(C) Binding of wild type Vav-3 to RhoA.	bind
11410	1	4525	5	NULL	NULL	0	NULL	Wnt8	NULL		bind	NULL				LRP6	NULL				NULL		0	NULL	NULL	NULL	gw70_development_130_18_4295_s_276	12900447	(C) Binding of Wnt8 and  LRP6 is attenuated in the presence of Wise, but binding of Wnt8 and Frizzled8 is  not.	bind
11411	2	4525	5	NULL	NULL	0	NULL	Wise	NULL	presence of	attenuate	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_development_130_18_4295_s_276	12900447	(C) Binding of Wnt8 and  LRP6 is attenuated in the presence of Wise, but binding of Wnt8 and Frizzled8 is  not.	bind
11412	3	4525	5	NULL	NULL	0	NULL	Wnt8	NULL		bind	NULL				Frizzled8	NULL				NULL		0	NULL	NULL	NULL	gw70_development_130_18_4295_s_276	12900447	(C) Binding of Wnt8 and  LRP6 is attenuated in the presence of Wise, but binding of Wnt8 and Frizzled8 is  not.	bind
11413	4	4525	5	NULL	NULL	0	NULL	Wise	NULL	presence of	does not attenuate	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_development_130_18_4295_s_276	12900447	(C) Binding of Wnt8 and  LRP6 is attenuated in the presence of Wise, but binding of Wnt8 and Frizzled8 is  not.	bind
11137	1	4525	6	NULL	NULL	NULL	NULL	Wnt8	GP		bind					LRP6	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_130_18_4295_s_276	12900447	(C) Binding of Wnt8 and  LRP6 is attenuated in the presence of Wise, but binding of Wnt8 and Frizzled8 is  not.	bind
11138	2	4525	6	NULL	NULL	NULL	NULL	Wise	GP		attenuates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_130_18_4295_s_276	12900447	(C) Binding of Wnt8 and  LRP6 is attenuated in the presence of Wise, but binding of Wnt8 and Frizzled8 is  not.	bind
11139	3	4525	6	NULL	NULL	NULL	NULL	Wnt8	GP		bind					Frizzled8	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_130_18_4295_s_276	12900447	(C) Binding of Wnt8 and  LRP6 is attenuated in the presence of Wise, but binding of Wnt8 and Frizzled8 is  not.	bind
11140	4	4525	6	NULL	NULL	NULL	NULL	wise	GP		does not attenuate					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_130_18_4295_s_276	12900447	(C) Binding of Wnt8 and  LRP6 is attenuated in the presence of Wise, but binding of Wnt8 and Frizzled8 is  not.	bind
11605	1	4527	5	NULL	NULL	0	NULL	RNAP	NULL	WT	bind	NULL				srf	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_12_4300_s_193	16740936	(C) Binding of WT and mutant  rpoA( C265A) RNAP with ComA P to the  srf promoter as determined by SPPR analysis.	bind
11606	2	4527	5	NULL	NULL	0	NULL	statement 1	NULL		occurs with	NULL				ComA P	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_12_4300_s_193	16740936	(C) Binding of WT and mutant  rpoA( C265A) RNAP with ComA P to the  srf promoter as determined by SPPR analysis.	bind
11607	3	4527	5	10	NULL	0	NULL	rpoA RNAP		mutant	bind			 C265A		srf				promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_12_4300_s_193	16740936	(C) Binding of WT and mutant  rpoA( C265A) RNAP with ComA P to the  srf promoter as determined by SPPR analysis.	bind
11608	4	4527	5	NULL	NULL	0	NULL	statement 3	NULL		occurs with	NULL				ComA P	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_12_4300_s_193	16740936	(C) Binding of WT and mutant  rpoA( C265A) RNAP with ComA P to the  srf promoter as determined by SPPR analysis.	bind
11141	1	4527	6	NULL	NULL	NULL	NULL	RNAP	GP	wild type	bind					srf	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_12_4300_s_193	16740936	(C) Binding of WT and mutant  rpoA( C265A) RNAP with ComA P to the  srf promoter as determined by SPPR analysis.	bind
11142	2	4527	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs with					ComA P	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_12_4300_s_193	16740936	(C) Binding of WT and mutant  rpoA( C265A) RNAP with ComA P to the  srf promoter as determined by SPPR analysis.	bind
11143	3	4527	6	NULL	NULL	NULL	NULL	rpoA RNAP	GP	mutant	bind			C265A		srf	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_12_4300_s_193	16740936	(C) Binding of WT and mutant  rpoA( C265A) RNAP with ComA P to the  srf promoter as determined by SPPR analysis.	bind
11144	4	4527	6	NULL	NULL	NULL	NULL	statement 3	Process		occurs with					ComA P	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_12_4300_s_193	16740936	(C) Binding of WT and mutant  rpoA( C265A) RNAP with ComA P to the  srf promoter as determined by SPPR analysis.	bind
11414	1	4528	5	NULL	NULL	0	NULL	BiP	NULL	wt	bind	NULL				Ig HC	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_3_921_s_95	15657421	(C) Binding of wt and mutant BiP to Ig HC and ATF6.	bind
11415	2	4528	5	NULL	NULL	0	NULL	BiP	NULL	mutant	bind	NULL				Ig HC	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_3_921_s_95	15657421	(C) Binding of wt and mutant BiP to Ig HC and ATF6.	bind
11416	3	4528	5	NULL	NULL	0	NULL	BiP	NULL	wt	bind	NULL				ATF6	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_3_921_s_95	15657421	(C) Binding of wt and mutant BiP to Ig HC and ATF6.	bind
11417	4	4528	5	NULL	NULL	0	NULL	BiP	NULL	mutant	bind	NULL				ATF6	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_3_921_s_95	15657421	(C) Binding of wt and mutant BiP to Ig HC and ATF6.	bind
11145	1	4528	6	NULL	NULL	NULL	NULL	BiP	GP	wild type	bind					Ig HC	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_3_921_s_95	15657421	(C) Binding of wt and mutant BiP to Ig HC and ATF6.	bind
11146	2	4528	6	NULL	NULL	0	NULL	BiP	NULL	mutant	bind	NULL				Ig HC	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_3_921_s_95	15657421	(C) Binding of wt and mutant BiP to Ig HC and ATF6.	bind
11147	3	4528	6	NULL	NULL	0	NULL	BiP	NULL	wild type	bind	NULL				ATF6	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_3_921_s_95	15657421	(C) Binding of wt and mutant BiP to Ig HC and ATF6.	bind
11148	4	4528	6	NULL	NULL	0	NULL	BiP	NULL	mutant	bind	NULL				ATF6	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_3_921_s_95	15657421	(C) Binding of wt and mutant BiP to Ig HC and ATF6.	bind
11419	1	4530	5	NULL	NULL	0	NULL		NULL		bind	NULL		CTD amino acids Y1-S7		Pin1	NULL		WW domain		NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_6_1549_s_162	12820968	(C) Blue ribbon representation of the backbone and solid bond representation for CTD amino acids Y1-S7 bound to the WW domain of Pin1 (PDB code 1f8a).	bind
11149	1	4530	6	NULL	NULL	NULL	NULL				bind			CTD amino acids Y1-S7		Pin1	GP		WW domain		NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_6_1549_s_162	12820968	(C) Blue ribbon representation of the backbone and solid bond representation for CTD amino acids Y1-S7 bound to the WW domain of Pin1 (PDB code 1f8a).	bind
11460	1	4531	5	NULL	NULL	0	NULL	endophilin	NULL		contains	NULL					NULL		NH2-terminus lipid binding region		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_2_193_s_84	11604418	(C) Both the NH2-terminal lipid binding region and the SH3 domain of endophilin (which binds dynamin) are required to form a complex of endophilin and dynamin on the lipid bilayer.	bind
11461	2	4531	5	NULL	NULL	0	NULL	endophilin	NULL		contains	NULL					NULL	 	SH3 domain dynamin binding region		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_2_193_s_84	11604418	(C) Both the NH2-terminal lipid binding region and the SH3 domain of endophilin (which binds dynamin) are required to form a complex of endophilin and dynamin on the lipid bilayer.	bind
11462	3	4531	5	10	NULL	0	NULL	endophilin	NULL		forms complex with	NULL				dynamin	NULL				NULL	lipid bilayer	NULL	NULL	NULL	NULL	gw60_cellbiol_155_2_193_s_84	11604418	(C) Both the NH2-terminal lipid binding region and the SH3 domain of endophilin (which binds dynamin) are required to form a complex of endophilin and dynamin on the lipid bilayer.	bind
11463	4	4531	5	10	NULL	0	NULL	statement 1	NULL		is required for	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_2_193_s_84	11604418	(C) Both the NH2-terminal lipid binding region and the SH3 domain of endophilin (which binds dynamin) are required to form a complex of endophilin and dynamin on the lipid bilayer.	bind
11464	5	4531	5	10	NULL	0	NULL	statement 2	NULL		is required for	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_2_193_s_84	11604418	(C) Both the NH2-terminal lipid binding region and the SH3 domain of endophilin (which binds dynamin) are required to form a complex of endophilin and dynamin on the lipid bilayer.	bind
11150	1	4531	6	NULL	NULL	NULL	NULL	endophilin	GP		contains								NH2-terminal lipid binding region		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_2_193_s_84	11604418	(C) Both the NH2-terminal lipid binding region and the SH3 domain of endophilin (which binds dynamin) are required to form a complex of endophilin and dynamin on the lipid bilayer.	bind
11151	2	4531	6	NULL	NULL	NULL	NULL	endophilin	GP		contains								SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_2_193_s_84	11604418	(C) Both the NH2-terminal lipid binding region and the SH3 domain of endophilin (which binds dynamin) are required to form a complex of endophilin and dynamin on the lipid bilayer.	bind
11152	3	4531	6	NULL	NULL	NULL	NULL	endophilin	GP		forms a complex with					dynamin	GP				NULL	lipid bilayer	NULL	NULL	NULL	NULL	gw60_cellbiol_155_2_193_s_84	11604418	(C) Both the NH2-terminal lipid binding region and the SH3 domain of endophilin (which binds dynamin) are required to form a complex of endophilin and dynamin on the lipid bilayer.	bind
54429	4	4531	6	NULL	NULL	NULL	NULL	statement 1	Process		is required for					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_2_193_s_84	11604418	(C) Both the NH2-terminal lipid binding region and the SH3 domain of endophilin (which binds dynamin) are required to form a complex of endophilin and dynamin on the lipid bilayer.	bind
54430	5	4531	6	NULL	NULL	NULL	NULL	statement 2	Process		is required for					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_2_193_s_84	11604418	(C) Both the NH2-terminal lipid binding region and the SH3 domain of endophilin (which binds dynamin) are required to form a complex of endophilin and dynamin on the lipid bilayer.	bind
11468	1	4533	5	NULL	NULL	0	NULL	USF	NULL		bind	NULL					NULL			E1-box	NULL	in non-HGF expressing cell types	0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_2_374_s_143	12163028	(C) But in non-HGF expressing cell types USF bound to the E1-box mediates gene repression supported by its interaction with an inhibitory transcriptional factor.	bind
11469	2	4533	5	NULL	NULL	0	NULL	statement 1	NULL		mediate	NULL				gene repression	NULL				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_2_374_s_143	12163028	(C) But in non-HGF expressing cell types USF bound to the E1-box mediates gene repression supported by its interaction with an inhibitory transcriptional factor.	bind
11470	3	4533	5	NULL	NULL	0	NULL	USF	NULL		interacts with	NULL				inhibitory transcriptional factor	NULL				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_2_374_s_143	12163028	(C) But in non-HGF expressing cell types USF bound to the E1-box mediates gene repression supported by its interaction with an inhibitory transcriptional factor.	bind
13131	4	4533	5	NULL	NULL	0	NULL	statement 2	NULL		is supported by	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_2_374_s_143	12163028	(C) But in non-HGF expressing cell types USF bound to the E1-box mediates gene repression supported by its interaction with an inhibitory transcriptional factor.	bind
11153	1	4533	6	NULL	NULL	NULL	NULL	USF	GP		bind									E1-box	NULL	non-HGF expressing cell types	NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_2_374_s_143	12163028	(C) But in non-HGF expressing cell types USF bound to the E1-box mediates gene repression supported by its interaction with an inhibitory transcriptional factor.	bind
11154	2	4533	6	NULL	NULL	NULL	NULL	USF	GP		interacts with					inhibitory transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_2_374_s_143	12163028	(C) But in non-HGF expressing cell types USF bound to the E1-box mediates gene repression supported by its interaction with an inhibitory transcriptional factor.	bind
12878	3	4533	6	NULL	NULL	NULL	NULL	statement 1	Process		mediates					gene expression	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_2_374_s_143	12163028	(C) But in non-HGF expressing cell types USF bound to the E1-box mediates gene repression supported by its interaction with an inhibitory transcriptional factor.	bind
13004	4	4533	6	NULL	NULL	NULL	NULL	statement 3	Process		is supported by					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_2_374_s_143	12163028	(C) But in non-HGF expressing cell types USF bound to the E1-box mediates gene repression supported by its interaction with an inhibitory transcriptional factor.	bind
11471	1	4534	5	NULL	NULL	0	NULL	C-Vps/HOPS proteins	NULL		bind	NULL				mon1delta vacuoles	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_163_5_973_s_69	14662743	(C) C-Vps/HOPS proteins are bound to the  mon1delta vacuoles.	bind
11155	1	4534	6	NULL	NULL	NULL	NULL	C-Vps/HOPS protein	GP		bind to					mon1delta vacuoles	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_163_5_973_s_69	14662743	(C) C-Vps/HOPS proteins are bound to the  mon1delta vacuoles.	bind
11472	2	4535	5	10	NULL	0	NULL	C4BP			does not bind					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_immunity_18_6_837_s_76	12818164	(C) C4BP and anti-CD40 fail to bind to B cells from a CD40-deficient patient.	bind
11473	2	4535	5	10	NULL	0	NULL	anti-CD40			does not bind					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_immunity_18_6_837_s_76	12818164	(C) C4BP and anti-CD40 fail to bind to B cells from a CD40-deficient patient.	bind
54431	1	4535	5	10	NULL	0	NULL	B cells 			derived from					CD40-deficient patient					NULL		0	NULL	NULL	NULL	gw60_immunity_18_6_837_s_76	12818164	(C) C4BP and anti-CD40 fail to bind to B cells from a CD40-deficient patient.	bind
11156	1	4535	6	NULL	NULL	NULL	NULL	B cells 	Cell		derived from					CD40 deficient patients	Person				NULL		NULL	NULL	NULL	NULL	gw60_immunity_18_6_837_s_76	12818164	(C) C4BP and anti-CD40 fail to bind to B cells from a CD40-deficient patient.	bind
11157	2	4535	6	NULL	NULL	NULL	NULL	C4BP	GP		does not bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_18_6_837_s_76	12818164	(C) C4BP and anti-CD40 fail to bind to B cells from a CD40-deficient patient.	bind
11158	3	4535	6	NULL	NULL	NULL	NULL	anti-CD40	GP		does not bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_18_6_837_s_76	12818164	(C) C4BP and anti-CD40 fail to bind to B cells from a CD40-deficient patient.	bind
11474	1	4537	5	NULL	NULL	0	NULL	CAND1	NULL		bind	NULL				CUL1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_10_6_1519_s_46	12504026	(C) CAND1 binding to CUL1 requires the carboxyl terminus of CUL1.	bind
11475	2	4537	5	NULL	NULL	0	NULL	statement 1	NULL		require	NULL				CUL1	NULL		carboxyl terminus		NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_6_1519_s_46	12504026	(C) CAND1 binding to CUL1 requires the carboxyl terminus of CUL1.	bind
11159	1	4537	6	NULL	NULL	NULL	NULL	CAND1	GP		bind					CUL1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_6_1519_s_46	12504026	(C) CAND1 binding to CUL1 requires the carboxyl terminus of CUL1.	bind
13005	2	4537	6	NULL	NULL	NULL	NULL	statement 1	Process		requires					CUL1	GP		carboxyl terminus of 		NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_6_1519_s_46	12504026	(C) CAND1 binding to CUL1 requires the carboxyl terminus of CUL1.	bind
11476	1	4538	5	NULL	NULL	0	NULL	CAS	NULL		bind	NULL	preferentially			importin	NULL	NLS-free			NULL		NULL	NULL	NULL	NULL	gw60_cell_90_6_1061_s_143	9323134	(C) CAS binds preferentially to NLS-free  importin  .	bind
11160	1	4538	6	NULL	NULL	NULL	NULL	CAS	GP		bind		preferentially			importin	GP	NLS free			NULL		NULL	NULL	NULL	NULL	gw60_cell_90_6_1061_s_143	9323134	(C) CAS binds preferentially to NLS-free  importin  .	bind
11477	1	4539	5	NULL	NULL	0	NULL	Cdc24	NULL		bind	NULL		N-terminal two-thirds		Pcn1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_2_1038_s_229	9891039	(C) Cdc24 binds Pcn1 and Rfc1 via its N-terminal two-thirds.	bind
11478	2	4539	5	NULL	NULL	0	NULL	Cdc24	NULL		bind	NULL		N-terminal two-thirds		Rfc1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_2_1038_s_229	9891039	(C) Cdc24 binds Pcn1 and Rfc1 via its N-terminal two-thirds.	bind
11161	1	4539	6	NULL	NULL	NULL	NULL	Cdc24	GP		bind			N-terminal two third		Pcn1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_2_1038_s_229	9891039	(C) Cdc24 binds Pcn1 and Rfc1 via its N-terminal two-thirds.	bind
11162	2	4539	6	NULL	NULL	NULL	NULL	Cdc24	GP		bind			N-terminal two third		Rfc1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_2_1038_s_229	9891039	(C) Cdc24 binds Pcn1 and Rfc1 via its N-terminal two-thirds.	bind
11479	1	4540	5	NULL	NULL	0	NULL	CDH1	NULL		bind	NULL				SnoN	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_8_5_1027_s_142	11741538	(C) CDH1 binds to SnoN in the presence of Smad3.	bind
11480	2	4540	5	NULL	NULL	0	NULL	statement 1	NULL		in the presence of	NULL				Smad3	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_8_5_1027_s_142	11741538	(C) CDH1 binds to SnoN in the presence of Smad3.	bind
11163	1	4540	6	NULL	NULL	NULL	NULL	CDH1	GP		bind					SnoN	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_5_1027_s_142	11741538	(C) CDH1 binds to SnoN in the presence of Smad3.	bind
11164	2	4540	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs in presence of					Smad3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_5_1027_s_142	11741538	(C) CDH1 binds to SnoN in the presence of Smad3.	bind
11483	1	4541	5	NULL	NULL	0	NULL	p53	NULL		bind	NULL				Apaf1	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_cellbiol_155_2_207_s_93	11591730	(C) Cell extracts (20 mug protein) obtained from untreated neurons or neurons exposed to camptothecin (10 muM) for 12 h were tested for p53 binding activity to the Apaf1 promoter elements as described above.	bind
54433	1	4541	6	NULL	NULL	NULL	NULL	p53	GP		bind					Apaf1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_2_207_s_93	11591730	(C) Cell extracts (20 mug protein) obtained from untreated neurons or neurons exposed to camptothecin (10 muM) for 12 h were tested for p53 binding activity to the Apaf1 promoter elements as described above.	bind
11484	1	4542	5	NULL	NULL	0	NULL	Pol II	NULL		bind	NULL					NULL			HS2	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_18_6484_s_105	12944475	(C) ChIP analysis of Pol II binding to HS2, HS3, and HS4, the active  Ey promoter, and intergenic site IVR5.	bind
11485	2	4542	5	NULL	NULL	0	NULL	Pol II	NULL		bind	NULL					NULL			HS3	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_18_6484_s_105	12944475	(C) ChIP analysis of Pol II binding to HS2, HS3, and HS4, the active  Ey promoter, and intergenic site IVR5.	bind
11486	3	4542	5	NULL	NULL	0	NULL	Pol II	NULL		bind	NULL					NULL			HS4	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_18_6484_s_105	12944475	(C) ChIP analysis of Pol II binding to HS2, HS3, and HS4, the active  Ey promoter, and intergenic site IVR5.	bind
11487	4	4542	5	NULL	NULL	0	NULL	Pol II	NULL		bind	NULL				Ey	NULL	active		promoter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_18_6484_s_105	12944475	(C) ChIP analysis of Pol II binding to HS2, HS3, and HS4, the active  Ey promoter, and intergenic site IVR5.	bind
11488	5	4542	5	NULL	NULL	0	NULL	Pol II	NULL		bind	NULL					NULL			intergenic site IVR5	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6484_s_105	12944475	(C) ChIP analysis of Pol II binding to HS2, HS3, and HS4, the active  Ey promoter, and intergenic site IVR5.	bind
11421	1	4542	6	10	NULL	0	NULL	Pol II			bind									HS2	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6484_s_105	12944475	(C) ChIP analysis of Pol II binding to HS2, HS3, and HS4, the active  Ey promoter, and intergenic site IVR5.	bind
11422	2	4542	6	10	NULL	0	NULL	Pol II			bind									HS3	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6484_s_105	12944475	(C) ChIP analysis of Pol II binding to HS2, HS3, and HS4, the active  Ey promoter, and intergenic site IVR5.	bind
11423	3	4542	6	10	NULL	0	NULL	Pol II			bind									HS4	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6484_s_105	12944475	(C) ChIP analysis of Pol II binding to HS2, HS3, and HS4, the active  Ey promoter, and intergenic site IVR5.	bind
11424	4	4542	6	NULL	NULL	0	NULL	Pol II	NULL		bind	NULL				Ey	NULL	active		promoter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_18_6484_s_105	12944475	(C) ChIP analysis of Pol II binding to HS2, HS3, and HS4, the active  Ey promoter, and intergenic site IVR5.	bind
11425	5	4542	6	NULL	NULL	0	NULL	Pol II	NULL		bind	NULL					NULL			intergenic site IVR5	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_18_6484_s_105	12944475	(C) ChIP analysis of Pol II binding to HS2, HS3, and HS4, the active  Ey promoter, and intergenic site IVR5.	bind
11489	1	4543	5	NULL	NULL	0	NULL	Rpb1	NULL		bind	NULL				GAL1	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_18_6270_s_213	11509669	(C) ChIP analysis of the binding of Rpb1 to the  GAL1 and  GAL10 promoters.	bind
11490	2	4543	5	NULL	NULL	0	NULL	Rpb1	NULL		bind	NULL				GAL10	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_18_6270_s_213	11509669	(C) ChIP analysis of the binding of Rpb1 to the  GAL1 and  GAL10 promoters.	bind
11426	1	4543	6	NULL	NULL	NULL	NULL	Rpb1	GP		bind					GAL1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_18_6270_s_213	11509669	(C) ChIP analysis of the binding of Rpb1 to the  GAL1 and  GAL10 promoters.	bind
11427	2	4543	6	NULL	NULL	NULL	NULL	Rpb1	GP		bind					GAL10	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_18_6270_s_213	11509669	(C) ChIP analysis of the binding of Rpb1 to the  GAL1 and  GAL10 promoters.	bind
11492	1	4544	5	NULL	NULL	0	NULL	Sox1	NULL		bind	NULL	directly			Hes1	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_devbiol_269_2_580_s_178	15110721	(C) ChIP assay demonstrates that Sox1 binds directly to the Hes1 promoter.	bind
11428	1	4544	6	NULL	NULL	NULL	NULL	Sox1	GP		bind		directly			Hes1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_devbiol_269_2_580_s_178	15110721	(C) ChIP assay demonstrates that Sox1 binds directly to the Hes1 promoter.	bind
11494	1	4545	5	NULL	NULL	0	NULL	MEF2	NULL		bind	NULL				 lklf	NULL			promoter	NULL	in vivo	0	NULL	NULL	NULL	gw70_molcellbiol_25_19_8553_s_303	16166637	(C) ChIP assays were performed to demonstrate in vivo binding of MEF2 to the  lklf promoter.	bind
11429	1	4545	6	NULL	NULL	NULL	NULL	MEF2	GP		bind					lklf	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8553_s_303	16166637	(C) ChIP assays were performed to demonstrate in vivo binding of MEF2 to the  lklf promoter.	bind
11495	1	4546	5	NULL	NULL	0	NULL	GATA-1	NULL		bind	NULL				TIMP-1	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_17_7412_s_142	16107690	(C) ChIP of GATA-1 bound to the  TIMP-1 promoter.	bind
11449	1	4546	6	NULL	NULL	NULL	NULL	GATA-1	GP		bind					TIMP-1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_17_7412_s_142	16107690	(C) ChIP of GATA-1 bound to the  TIMP-1 promoter.	bind
11497	1	4547	5	NULL	NULL	0	NULL	chPER3	NULL		bind	NULL				CKI	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_2_584_s_144	14701732	(C) chPER3 binds to CKI  more efficiently than mPER3, whereas chPER2 binds to CKI  much less efficiently than mPER2.	bind
11498	2	4547	5	NULL	NULL	0	NULL	mPER3	NULL		bind	NULL				CKI	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_2_584_s_144	14701732	(C) chPER3 binds to CKI  more efficiently than mPER3, whereas chPER2 binds to CKI  much less efficiently than mPER2.	bind
11500	3	4547	5	NULL	NULL	0	NULL	statement 1	NULL		is more efficient than	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_2_584_s_144	14701732	(C) chPER3 binds to CKI  more efficiently than mPER3, whereas chPER2 binds to CKI  much less efficiently than mPER2.	bind
11501	4	4547	5	NULL	NULL	0	NULL	chPER2	NULL		bind	NULL				CKI	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_2_584_s_144	14701732	(C) chPER3 binds to CKI  more efficiently than mPER3, whereas chPER2 binds to CKI  much less efficiently than mPER2.	bind
11503	5	4547	5	NULL	NULL	0	NULL	mPER2	NULL		bind	NULL				CKI	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_2_584_s_144	14701732	(C) chPER3 binds to CKI  more efficiently than mPER3, whereas chPER2 binds to CKI  much less efficiently than mPER2.	bind
11504	6	4547	5	NULL	NULL	0	NULL	statement 4	NULL		is less efficient than	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_2_584_s_144	14701732	(C) chPER3 binds to CKI  more efficiently than mPER3, whereas chPER2 binds to CKI  much less efficiently than mPER2.	bind
11450	1	4547	6	NULL	NULL	NULL	NULL	chPER3	GP		bind					CKI	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_2_584_s_144	14701732	(C) chPER3 binds to CKI  more efficiently than mPER3, whereas chPER2 binds to CKI  much less efficiently than mPER2.	bind
11451	2	4547	6	NULL	NULL	NULL	NULL	mPER3	GP		bind					CKI	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_2_584_s_144	14701732	(C) chPER3 binds to CKI  more efficiently than mPER3, whereas chPER2 binds to CKI  much less efficiently than mPER2.	bind
11452	3	4547	6	NULL	NULL	NULL	NULL	statement 1	Process		is more efficient than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_2_584_s_144	14701732	(C) chPER3 binds to CKI  more efficiently than mPER3, whereas chPER2 binds to CKI  much less efficiently than mPER2.	bind
11453	4	4547	6	NULL	NULL	NULL	NULL	chPER2	GP		bind					CKI	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_2_584_s_144	14701732	(C) chPER3 binds to CKI  more efficiently than mPER3, whereas chPER2 binds to CKI  much less efficiently than mPER2.	bind
11454	5	4547	6	NULL	NULL	NULL	NULL	mPER2	GP		bind					CKI	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_2_584_s_144	14701732	(C) chPER3 binds to CKI  more efficiently than mPER3, whereas chPER2 binds to CKI  much less efficiently than mPER2.	bind
11455	6	4547	6	NULL	NULL	NULL	NULL	statement 4	Process		is less efficient than					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_2_584_s_144	14701732	(C) chPER3 binds to CKI  more efficiently than mPER3, whereas chPER2 binds to CKI  much less efficiently than mPER2.	bind
11507	1	4549	5	NULL	NULL	0	NULL	Tcf3	NULL		bind	NULL				beta-catenin	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_154_5_983_s_217	11524435	(C) CK1epsilon stimulates the binding of Tcf3 to beta-catenin.	bind
11508	2	4549	5	NULL	NULL	0	NULL	CK1epsilon	NULL		stimulate	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_154_5_983_s_217	11524435	(C) CK1epsilon stimulates the binding of Tcf3 to beta-catenin.	bind
11456	1	4549	6	NULL	NULL	NULL	NULL	Tcf3	GP		bind					beta-catenin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_983_s_217	11524435	(C) CK1epsilon stimulates the binding of Tcf3 to beta-catenin.	bind
11457	2	4549	6	NULL	NULL	NULL	NULL	CK1epsilon	GP		stimulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_983_s_217	11524435	(C) CK1epsilon stimulates the binding of Tcf3 to beta-catenin.	bind
11510	1	4553	5	NULL	NULL	0	NULL	LR974P	NULL		bind	NULL				SHP-2	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1545_1_20_s_146	11342028	(C) Comparison of binding of LR986P and LR974P to SHP-2.	bind
11511	2	4553	5	NULL	NULL	0	NULL	LR986P	NULL		bind	NULL				SHP-2	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1545_1_20_s_146	11342028	(C) Comparison of binding of LR986P and LR974P to SHP-2.	bind
11458	1	4553	6	NULL	NULL	NULL	NULL	LR974P			bind					SHP-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1545_1_20_s_146	11342028	(C) Comparison of binding of LR986P and LR974P to SHP-2.	bind
11459	2	4553	6	NULL	NULL	NULL	NULL	LR986P			bind					SHP-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1545_1_20_s_146	11342028	(C) Comparison of binding of LR986P and LR974P to SHP-2.	bind
11600	1	4554	6	NULL	NULL	NULL	NULL	MAb9E			bind					MYC epitope	AminoAcid		C terminus of the intracellular domain		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_7_1709_s_146	9658166	(C) Comparison of Delta isoforms immunoprecipitated using MAb8A from cultured cells that express DeltaWTNdeMYC (lane 1) with Delta isoforms immunoprecipitated from DeltaWTNdeMYC+ cells with MAb9E, which binds to the MYC epitope at the C terminus of the intracellular domain (lane 2).	bind
11514	1	4555	5	10	NULL	0	NULL	Translin		 rat;; liver	bind									Bcl-CL1	NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1624_1_29_s_157	14642810	(C) Comparison of expressed rat liver Translin binding  to Bcl-CL1 and GRE (MLTF-like site) DNA.	bind
11515	2	4555	5	10	NULL	0	NULL	Translin		 rat;;liver	bind					DNA				GRE (MLTF-like site)	NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1624_1_29_s_157	14642810	(C) Comparison of expressed rat liver Translin binding  to Bcl-CL1 and GRE (MLTF-like site) DNA.	bind
11481	1	4555	6	NULL	NULL	NULL	NULL	translin	GP	rat;; liver	bind									Bcl-CL1	NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1624_1_29_s_157	14642810	(C) Comparison of expressed rat liver Translin binding  to Bcl-CL1 and GRE (MLTF-like site) DNA.	bind
11482	2	4555	6	NULL	NULL	NULL	NULL	translin	GP	rat;; liver	bind					DNA	NucleicAcid			GRE (MLTF-like site)	NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1624_1_29_s_157	14642810	(C) Comparison of expressed rat liver Translin binding  to Bcl-CL1 and GRE (MLTF-like site) DNA.	bind
11517	1	4557	5	NULL	NULL	0	NULL	MEKK-1	NULL		phosphorylate	NULL				SMRT	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_17_6612_s_250	10938135	(C) Comparison of MEKK-1 phosphorylation of SMRT and of SEK-1.	bind
11518	2	4557	5	NULL	NULL	0	NULL	MEKK-1	NULL		phosphorylate	NULL				SEK-1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_17_6612_s_250	10938135	(C) Comparison of MEKK-1 phosphorylation of SMRT and of SEK-1.	bind
11491	1	4557	6	NULL	NULL	NULL	NULL	MEKK-1	GP		phosphorylates					SMRT	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6612_s_250	10938135	(C) Comparison of MEKK-1 phosphorylation of SMRT and of SEK-1.	bind
11493	2	4557	6	NULL	NULL	NULL	NULL	MEKK-1	GP		phosphorylates					SEK-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6612_s_250	10938135	(C) Comparison of MEKK-1 phosphorylation of SMRT and of SEK-1.	bind
11519	1	4558	5	NULL	NULL	0	NULL	PP1c	NULL		bind	NULL				AKAP220 peptide	NULL	human			NULL		0	NULL	NULL	NULL	gw60_currbiol_9_6_321_s_53	10209101	(c) Comparison of PP1c  binding to the human AKAP220 peptide, the rat AKAP220 peptide, and the GM subunit peptide ( plus-or-minus  standard error).	bind
11520	2	4558	5	NULL	NULL	0	NULL	PP1c	NULL		bind	NULL				AKAP220 peptide	NULL	rat			NULL		0	NULL	NULL	NULL	gw60_currbiol_9_6_321_s_53	10209101	(c) Comparison of PP1c  binding to the human AKAP220 peptide, the rat AKAP220 peptide, and the GM subunit peptide ( plus-or-minus  standard error).	bind
11521	3	4558	5	NULL	NULL	0	NULL	PP1c	NULL		bind	NULL				GM subunit peptide	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_9_6_321_s_53	10209101	(c) Comparison of PP1c  binding to the human AKAP220 peptide, the rat AKAP220 peptide, and the GM subunit peptide ( plus-or-minus  standard error).	bind
11496	1	4558	6	NULL	NULL	NULL	NULL	PP1c	GP		bind					AKAP220 peptide	AminoAcid	human			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_6_321_s_53	10209101	(c) Comparison of PP1c  binding to the human AKAP220 peptide, the rat AKAP220 peptide, and the GM subunit peptide ( plus-or-minus  standard error).	bind
11499	2	4558	6	NULL	NULL	NULL	NULL	PP1c	GP		bind					AKAP220 peptide	AminoAcid	rat			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_6_321_s_53	10209101	(c) Comparison of PP1c  binding to the human AKAP220 peptide, the rat AKAP220 peptide, and the GM subunit peptide ( plus-or-minus  standard error).	bind
11502	3	4558	6	NULL	NULL	NULL	NULL	PP1c	GP		bind					GM subunit peptide	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_9_6_321_s_53	10209101	(c) Comparison of PP1c  binding to the human AKAP220 peptide, the rat AKAP220 peptide, and the GM subunit peptide ( plus-or-minus  standard error).	bind
11522	1	4559	5	NULL	NULL	0	NULL	JNK isoform	NULL	human	bind	NULL				JIP1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_10_7245_s_166	10490659	(C) Comparison of the binding of 10 human JNK isoforms to JIP1 and JIP2.	bind
11523	2	4559	5	NULL	NULL	0	NULL	JNK isoform	NULL	human	bind	NULL				JIP2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_10_7245_s_166	10490659	(C) Comparison of the binding of 10 human JNK isoforms to JIP1 and JIP2.	bind
11505	1	4559	6	NULL	NULL	NULL	NULL	JNK isoforms	GP	human	bind					JIP1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_7245_s_166	10490659	(C) Comparison of the binding of 10 human JNK isoforms to JIP1 and JIP2.	bind
11506	2	4559	6	NULL	NULL	NULL	NULL	JNK isoforms	GP	human	bind					JIP2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_7245_s_166	10490659	(C) Comparison of the binding of 10 human JNK isoforms to JIP1 and JIP2.	bind
11524	1	4560	5	NULL	NULL	0	NULL	JNK isoform	NULL		bind	NULL				JIP3	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_3_1030_s_160	10629060	(C) Comparison of the binding of 10 JNK isoforms to JIP3.	bind
11509	1	4560	6	NULL	NULL	NULL	NULL	JNK isoforms	GP		bind					JIP3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_3_1030_s_160	10629060	(C) Comparison of the binding of 10 JNK isoforms to JIP3.	bind
11525	1	4561	5	NULL	NULL	0	NULL	TBL1	NULL		bind	NULL	preferentially			histones	NULL	hypoacetylated			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_1_324_s_197	15601853	(C) Competition  experiments showing that TBL1 and TBLR1 bound preferentially to hypoacetylated histones.	bind
11526	2	4561	5	NULL	NULL	0	NULL	TBLR1	NULL		bind	NULL	preferentially			histones	NULL	hypoacetylated			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_1_324_s_197	15601853	(C) Competition  experiments showing that TBL1 and TBLR1 bound preferentially to hypoacetylated histones.	bind
11512	1	4561	6	NULL	NULL	NULL	NULL	TBL1	GP		bind		preferentially			histones	GP	hypoacetylated			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_1_324_s_197	15601853	(C) Competition  experiments showing that TBL1 and TBLR1 bound preferentially to hypoacetylated histones.	bind
11513	2	4561	6	NULL	NULL	NULL	NULL	TBLR1	GP		bind		preferentially			histones	GP	hypoacetylated			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_1_324_s_197	15601853	(C) Competition  experiments showing that TBL1 and TBLR1 bound preferentially to hypoacetylated histones.	bind
11527	1	4562	5	NULL	NULL	0	NULL	tRNAAla	NULL	unlabeled	bind	NULL				mitochondria	NULL	isolated			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_11_4000_s_243	12748301	(C) Competition experiments of tRNAAla binding onto isolated mitochondria using unlabeled tRNAAla, tRNAPhe, or tRNAMet-e as competitors.	bind
11528	2	4562	5	NULL	NULL	0	NULL	tRNAPhe	NULL	unlabeled	bind	NULL				mitochondria	NULL	isolated			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_11_4000_s_243	12748301	(C) Competition experiments of tRNAAla binding onto isolated mitochondria using unlabeled tRNAAla, tRNAPhe, or tRNAMet-e as competitors.	bind
11529	3	4562	5	NULL	NULL	0	NULL	tRNAMet-e	NULL	unlabeled	bind	NULL				mitochondria	NULL	isolated			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_11_4000_s_243	12748301	(C) Competition experiments of tRNAAla binding onto isolated mitochondria using unlabeled tRNAAla, tRNAPhe, or tRNAMet-e as competitors.	bind
11530	4	4562	5	NULL	NULL	0	NULL	statement 2	NULL		compete with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_11_4000_s_243	12748301	(C) Competition experiments of tRNAAla binding onto isolated mitochondria using unlabeled tRNAAla, tRNAPhe, or tRNAMet-e as competitors.	bind
11531	5	4562	5	NULL	NULL	0	NULL	statement 3	NULL		compete with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_11_4000_s_243	12748301	(C) Competition experiments of tRNAAla binding onto isolated mitochondria using unlabeled tRNAAla, tRNAPhe, or tRNAMet-e as competitors.	bind
11547	1	4562	6	NULL	NULL	NULL	NULL	tRNAAla	NucleicAcid		bind					mitochondria	CellComponent	isolated			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_11_4000_s_243	12748301	(C) Competition experiments of tRNAAla binding onto isolated mitochondria using unlabeled tRNAAla, tRNAPhe, or tRNAMet-e as competitors.	bind
11548	2	4562	6	NULL	NULL	NULL	NULL	tRNAAla	NucleicAcid	unlabeled	bind					mitochondria	CellComponent	isolated			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_11_4000_s_243	12748301	(C) Competition experiments of tRNAAla binding onto isolated mitochondria using unlabeled tRNAAla, tRNAPhe, or tRNAMet-e as competitors.	bind
11549	3	4562	6	NULL	NULL	NULL	NULL	statement 2	Process		competes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_11_4000_s_243	12748301	(C) Competition experiments of tRNAAla binding onto isolated mitochondria using unlabeled tRNAAla, tRNAPhe, or tRNAMet-e as competitors.	bind
11550	4	4562	6	NULL	NULL	NULL	NULL	tRNAPhe	NucleicAcid	unlabeled	bind					mitochondria	CellComponent	isolated			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_11_4000_s_243	12748301	(C) Competition experiments of tRNAAla binding onto isolated mitochondria using unlabeled tRNAAla, tRNAPhe, or tRNAMet-e as competitors.	bind
11551	5	4562	6	NULL	NULL	NULL	NULL	statement 4	Process		competes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_11_4000_s_243	12748301	(C) Competition experiments of tRNAAla binding onto isolated mitochondria using unlabeled tRNAAla, tRNAPhe, or tRNAMet-e as competitors.	bind
11552	6	4562	6	NULL	NULL	NULL	NULL	tRNAMet-e	NucleicAcid	unlabeled	bind					mitochondria	CellComponent	isolated			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_11_4000_s_243	12748301	(C) Competition experiments of tRNAAla binding onto isolated mitochondria using unlabeled tRNAAla, tRNAPhe, or tRNAMet-e as competitors.	bind
11553	7	4562	6	NULL	NULL	NULL	NULL	statement 6	Process		competes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_11_4000_s_243	12748301	(C) Competition experiments of tRNAAla binding onto isolated mitochondria using unlabeled tRNAAla, tRNAPhe, or tRNAMet-e as competitors.	bind
11532	1	4563	5	NULL	NULL	0	NULL	NF D	NULL		bind	NULL				rDNA probe A123BP	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_16_7284_s_178	15282326	(C) Competition for binding of NF D to rDNA probe A123BP with increasing amounts of unlabeled rDNA A123BP or rA123BPH as indicated.	bind
11533	2	4563	5	NULL	NULL	0	NULL	NF D	NULL		bind	NULL				rDNA A123BP	NULL	unlabeled			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_16_7284_s_178	15282326	(C) Competition for binding of NF D to rDNA probe A123BP with increasing amounts of unlabeled rDNA A123BP or rA123BPH as indicated.	bind
11534	3	4563	5	NULL	NULL	0	NULL	NF D	NULL		bind	NULL				rA123BPH	NULL	unlabeled			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_16_7284_s_178	15282326	(C) Competition for binding of NF D to rDNA probe A123BP with increasing amounts of unlabeled rDNA A123BP or rA123BPH as indicated.	bind
11535	4	4563	5	NULL	NULL	0	NULL	statement 2	NULL		compete with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_16_7284_s_178	15282326	(C) Competition for binding of NF D to rDNA probe A123BP with increasing amounts of unlabeled rDNA A123BP or rA123BPH as indicated.	bind
11536	5	4563	5	NULL	NULL	0	NULL	statement 3	NULL		compete with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_16_7284_s_178	15282326	(C) Competition for binding of NF D to rDNA probe A123BP with increasing amounts of unlabeled rDNA A123BP or rA123BPH as indicated.	bind
54436	6	4563	5	10	NULL	0	NULL	statement 2			is an alternative to					statement 3					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_16_7284_s_178	15282326	(C) Competition for binding of NF D to rDNA probe A123BP with increasing amounts of unlabeled rDNA A123BP or rA123BPH as indicated.	bind
11554	1	4563	6	NULL	NULL	NULL	NULL	NF D			bind					rDNA A123BP	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_16_7284_s_178	15282326	(C) Competition for binding of NF D to rDNA probe A123BP with increasing amounts of unlabeled rDNA A123BP or rA123BPH as indicated.	bind
11555	2	4563	6	NULL	NULL	NULL	NULL	NF D			bind					rDNA A123BP	NucleicAcid	unlabeled			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_16_7284_s_178	15282326	(C) Competition for binding of NF D to rDNA probe A123BP with increasing amounts of unlabeled rDNA A123BP or rA123BPH as indicated.	bind
11556	3	4563	6	NULL	NULL	NULL	NULL	statement 1	Process		competes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_16_7284_s_178	15282326	(C) Competition for binding of NF D to rDNA probe A123BP with increasing amounts of unlabeled rDNA A123BP or rA123BPH as indicated.	bind
11557	4	4563	6	NULL	NULL	NULL	NULL	NF D			bind					rDNA A123BPH	NucleicAcid	unlabeled			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_16_7284_s_178	15282326	(C) Competition for binding of NF D to rDNA probe A123BP with increasing amounts of unlabeled rDNA A123BP or rA123BPH as indicated.	bind
11558	5	4563	6	NULL	NULL	NULL	NULL	statement 1	Process		competes					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_16_7284_s_178	15282326	(C) Competition for binding of NF D to rDNA probe A123BP with increasing amounts of unlabeled rDNA A123BP or rA123BPH as indicated.	bind
11559	6	4563	6	NULL	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_16_7284_s_178	15282326	(C) Competition for binding of NF D to rDNA probe A123BP with increasing amounts of unlabeled rDNA A123BP or rA123BPH as indicated.	bind
11537	1	4564	5	NULL	NULL	0	NULL	KKLF	NULL		bind	NULL					NULL			GA element	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_19_7319_s_142	10982849	(C) Competitive binding of KKLF and MAZ at the GA element.	bind
11538	2	4564	5	NULL	NULL	0	NULL	MAZ	NULL		bind	NULL					NULL			GA element	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_19_7319_s_142	10982849	(C) Competitive binding of KKLF and MAZ at the GA element.	bind
11539	3	4564	5	NULL	NULL	0	NULL	statement 1	NULL		compete with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_19_7319_s_142	10982849	(C) Competitive binding of KKLF and MAZ at the GA element.	bind
11560	1	4564	6	NULL	NULL	NULL	NULL	KKLF	GP		bind									GA element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7319_s_142	10982849	(C) Competitive binding of KKLF and MAZ at the GA element.	bind
11561	2	4564	6	NULL	NULL	NULL	NULL	MAZ	GP		bind									GA element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7319_s_142	10982849	(C) Competitive binding of KKLF and MAZ at the GA element.	bind
11562	3	4564	6	NULL	NULL	NULL	NULL	statement 1	Process		competes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7319_s_142	10982849	(C) Competitive binding of KKLF and MAZ at the GA element.	bind
11540	1	4566	5	NULL	NULL	0	NULL	Gsp1	NULL		bind	NULL				GTP	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_12_4295_s_221	10825193	(C) Complex formation is dependent on the GTP-bound form of Gsp1.	bind
11541	2	4566	5	NULL	NULL	0	NULL	complex formation	NULL		is dependent on	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_12_4295_s_221	10825193	(C) Complex formation is dependent on the GTP-bound form of Gsp1.	bind
11563	1	4566	6	NULL	NULL	NULL	NULL	Gsp1	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4295_s_221	10825193	(C) Complex formation is dependent on the GTP-bound form of Gsp1.	bind
11542	1	4567	5	NULL	NULL	0	NULL	syntaxin-1A	NULL		bind	NULL				myosin-Va	NULL				NULL	in brain homogenate (Crude)	0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_94	16030255	(C) Confirmation of the 10 - 6 M Ca2+/2 mM Mg2+/0.5 mM ATP-dependent binding of syntaxin-1A to myosin-Va in brain homogenate (Crude)  or to purified myosin-Va (Purified).	bind
11543	2	4567	5	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_94	16030255	(C) Confirmation of the 10 - 6 M Ca2+/2 mM Mg2+/0.5 mM ATP-dependent binding of syntaxin-1A to myosin-Va in brain homogenate (Crude)  or to purified myosin-Va (Purified).	bind
11544	3	4567	5	NULL	NULL	0	NULL	syntaxin-1A	NULL		bind	NULL				myosin-Va	NULL	purified			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_94	16030255	(C) Confirmation of the 10 - 6 M Ca2+/2 mM Mg2+/0.5 mM ATP-dependent binding of syntaxin-1A to myosin-Va in brain homogenate (Crude)  or to purified myosin-Va (Purified).	bind
11545	4	4567	5	NULL	NULL	0	NULL	statement 3	NULL		is dependent on	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_94	16030255	(C) Confirmation of the 10 - 6 M Ca2+/2 mM Mg2+/0.5 mM ATP-dependent binding of syntaxin-1A to myosin-Va in brain homogenate (Crude)  or to purified myosin-Va (Purified).	bind
11546	5	4567	5	NULL	NULL	0	NULL	statement 4	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_94	16030255	(C) Confirmation of the 10 - 6 M Ca2+/2 mM Mg2+/0.5 mM ATP-dependent binding of syntaxin-1A to myosin-Va in brain homogenate (Crude)  or to purified myosin-Va (Purified).	bind
11564	1	4567	6	NULL	NULL	NULL	NULL	syntaxin-1A	GP		bind					myosin-Va	GP				NULL	brain homogenate	NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_94	16030255	(C) Confirmation of the 10 - 6 M Ca2+/2 mM Mg2+/0.5 mM ATP-dependent binding of syntaxin-1A to myosin-Va in brain homogenate (Crude)  or to purified myosin-Va (Purified).	bind
11565	2	4567	6	NULL	NULL	NULL	NULL	syntaxin-1A	GP		bind					myosin-Va	GP	purified			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_94	16030255	(C) Confirmation of the 10 - 6 M Ca2+/2 mM Mg2+/0.5 mM ATP-dependent binding of syntaxin-1A to myosin-Va in brain homogenate (Crude)  or to purified myosin-Va (Purified).	bind
11566	3	4567	6	NULL	NULL	NULL	NULL	statement 1	Process		is dependent on					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_94	16030255	(C) Confirmation of the 10 - 6 M Ca2+/2 mM Mg2+/0.5 mM ATP-dependent binding of syntaxin-1A to myosin-Va in brain homogenate (Crude)  or to purified myosin-Va (Purified).	bind
11567	4	4567	6	NULL	NULL	NULL	NULL	statement 2	Process		is dependent on					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_94	16030255	(C) Confirmation of the 10 - 6 M Ca2+/2 mM Mg2+/0.5 mM ATP-dependent binding of syntaxin-1A to myosin-Va in brain homogenate (Crude)  or to purified myosin-Va (Purified).	bind
54437	5	4567	6	NULL	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_94	16030255	(C) Confirmation of the 10 - 6 M Ca2+/2 mM Mg2+/0.5 mM ATP-dependent binding of syntaxin-1A to myosin-Va in brain homogenate (Crude)  or to purified myosin-Va (Purified).	bind
11614	1	4569	5	10	NULL	0	NULL	methyltransferase	NULL		bind	NULL		HsdM subunits			NULL		linker region		NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_64_2_412_s_131	10839821	(c) Consequent model of the methyltransferase, in which the two HsdM subunits bind  to the linker region to generate an enzyme with pseudodyad symmetry.	bind
11615	2	4569	5	NULL	NULL	0	NULL	statement 1	NULL		generate	NULL				enzyme	NULL	 pseudodyad symmetry			NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_64_2_412_s_131	10839821	(c) Consequent model of the methyltransferase, in which the two HsdM subunits bind  to the linker region to generate an enzyme with pseudodyad symmetry.	bind
11568	1	4569	6	NULL	NULL	NULL	NULL	methyltransferase	GP		bind			HsdM subunits					linker region		NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_64_2_412_s_131	10839821	(c) Consequent model of the methyltransferase, in which the two HsdM subunits bind  to the linker region to generate an enzyme with pseudodyad symmetry.	bind
11569	2	4569	6	NULL	NULL	NULL	NULL	statement 1	Process		generates					enzyme	GP	pseudodyad symmetry			NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_64_2_412_s_131	10839821	(c) Consequent model of the methyltransferase, in which the two HsdM subunits bind  to the linker region to generate an enzyme with pseudodyad symmetry.	bind
11609	1	4571	5	NULL	NULL	0	NULL	Vera	NULL		bind	NULL				E2	NULL	deletion mutants			NULL		0	NULL	NULL	NULL	gw60_currbiol_8_9_489_s_60	9560341	(c) Correlation between localization  in vivo and Vera binding of E2 deletion mutants.	bind
11570	1	4571	6	NULL	NULL	NULL	NULL	E2	GP	deletion mutant	bind					Vera	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_9_489_s_60	9560341	(c) Correlation between localization  in vivo and Vera binding of E2 deletion mutants.	bind
11610	1	4573	5	NULL	NULL	0	NULL	VEGFR2	NULL		bind	NULL	selectively			F-actin	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_267_2_294_s_182	15013795	(C) Costaining for VEGFR2 (green) and phalloidin-Alexa Fluor 568 (red), which binds  to F-actin selectively and delineates the myocardium.	bind
11611	2	4573	5	NULL	NULL	0	NULL	VEGFR2	NULL		delineates	NULL				myocardium	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_267_2_294_s_182	15013795	(C) Costaining for VEGFR2 (green) and phalloidin-Alexa Fluor 568 (red), which binds  to F-actin selectively and delineates the myocardium.	bind
11612	3	4573	5	NULL	NULL	0	NULL	phalloidin-Alexa Fluor 568	NULL		bind	NULL	selectively			F-actin	NULL				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_267_2_294_s_182	15013795	(C) Costaining for VEGFR2 (green) and phalloidin-Alexa Fluor 568 (red), which binds  to F-actin selectively and delineates the myocardium.	bind
11613	4	4573	5	NULL	NULL	0	NULL	statement 3	NULL		delineates	NULL				myocardium	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_267_2_294_s_182	15013795	(C) Costaining for VEGFR2 (green) and phalloidin-Alexa Fluor 568 (red), which binds  to F-actin selectively and delineates the myocardium.	bind
54438	1	4573	6	NULL	NULL	NULL	NULL	VEGFR2	GP		bind		selectively			F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_267_2_294_s_182	15013795	(C) Costaining for VEGFR2 (green) and phalloidin-Alexa Fluor 568 (red), which binds  to F-actin selectively and delineates the myocardium.	bind
54439	2	4573	6	NULL	NULL	NULL	NULL	statement 1	Process		delineates					myocardium	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_267_2_294_s_182	15013795	(C) Costaining for VEGFR2 (green) and phalloidin-Alexa Fluor 568 (red), which binds  to F-actin selectively and delineates the myocardium.	bind
11616	1	4574	5	NULL	NULL	0	NULL	MyoD	NULL	cotransfection of	does not alter	NULL				myogenin-positive cells	NULL	number of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_17_6600_s_197	10938134	(C) Cotransfection of MyoD and calcineurin (CnA) also does not alter the number of myogenin-positive cells.	bind
11617	2	4574	5	NULL	NULL	0	NULL	calcineurin (CnA)	NULL	cotransfection of	does not alter	NULL				myogenin-positive cells	NULL	number of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_17_6600_s_197	10938134	(C) Cotransfection of MyoD and calcineurin (CnA) also does not alter the number of myogenin-positive cells.	bind
16268	1	4574	6	NULL	NULL	NULL	NULL	MyoD	GP	cotransfection of	does not alter					myogenin-positive cells	Cell	number of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6600_s_197	10938134	(C) Cotransfection of MyoD and calcineurin (CnA) also does not alter the number of myogenin-positive cells.	bind
16269	2	4574	6	NULL	NULL	NULL	NULL	calcineurin (CnA)	GP	cotransfection of	does not alter					myogenin-positive cells	Cell	number of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6600_s_197	10938134	(C) Cotransfection of MyoD and calcineurin (CnA) also does not alter the number of myogenin-positive cells.	bind
11618	1	4575	5	NULL	NULL	0	NULL	CPR	NULL		bind	NULL				10-mer peptides	NULL				NULL	cellulose membrane	NULL	NULL	NULL	NULL	gw60_chembiol_9_10_1129_s_110	12401497	(C) CPR binding to PCI-derived 10-mer peptides on a cellulose membrane.	bind
44562	2	4575	5	10	NULL	0	NULL	10-mer peptides	NULL		is derived from	NULL				PCI	NULL				NULL		0	NULL	NULL	NULL	gw60_chembiol_9_10_1129_s_110	12401497	(C) CPR binding to PCI-derived 10-mer peptides on a cellulose membrane.	bind
11574	2	4575	6	NULL	NULL	NULL	NULL	CPR	GP		bind					statement 1	Process				NULL	cellulose membrane	NULL	NULL	NULL	NULL	gw60_chembiol_9_10_1129_s_110	12401497	(C) CPR binding to PCI-derived 10-mer peptides on a cellulose membrane.	bind
54440	1	4575	6	NULL	NULL	NULL	NULL	10-mer peptides	AminoAcid		derived from					PCI	GP				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_9_10_1129_s_110	12401497	(C) CPR binding to PCI-derived 10-mer peptides on a cellulose membrane.	bind
11619	1	4576	5	NULL	NULL	0	NULL	CREB	NULL		bind	NULL				cyclin D1	NULL			CRE of promoter	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_17_7514_s_218	15314161	(C) CREB and ATF-2 bind the CRE  of the cyclin D1 promoter.	bind
11620	2	4576	5	NULL	NULL	0	NULL	ATF-2	NULL		bind	NULL				cyclin D1	NULL			CRE of promoter	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_17_7514_s_218	15314161	(C) CREB and ATF-2 bind the CRE  of the cyclin D1 promoter.	bind
11575	1	4576	6	NULL	NULL	NULL	NULL	CREB	GP		bind					cyclin D1	GP			CRE element of promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_17_7514_s_218	15314161	(C) CREB and ATF-2 bind the CRE  of the cyclin D1 promoter.	bind
11576	2	4576	6	NULL	NULL	NULL	NULL	ATF-2	GP		bind					cyclin D1	GP			CRE element of promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_17_7514_s_218	15314161	(C) CREB and ATF-2 bind the CRE  of the cyclin D1 promoter.	bind
11621	1	4578	5	NULL	NULL	0	NULL	CSP	NULL		bind	NULL	dose dependently			Syntaxin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuron_23_3_593_s_218	10433270	(C) CSP binds Syntaxin in a dose-dependent and saturable manner.	bind
11623	2	4578	5	NULL	NULL	0	NULL	statement 1	NULL		occurs in	NULL				saturable manner	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuron_23_3_593_s_218	10433270	(C) CSP binds Syntaxin in a dose-dependent and saturable manner.	bind
11577	1	4578	6	NULL	NULL	NULL	NULL	CSP	GP		bind		dose dependently			Syntaxin	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_23_3_593_s_218	10433270	(C) CSP binds Syntaxin in a dose-dependent and saturable manner.	bind
16270	2	4578	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs in					saturable manner					NULL		NULL	NULL	NULL	NULL	gw60_neuron_23_3_593_s_218	10433270	(C) CSP binds Syntaxin in a dose-dependent and saturable manner.	bind
11624	1	4579	5	NULL	NULL	0	NULL	Tg	NULL		bind	NULL				BiP	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_22_9793_s_263	16260597	(C) CST causes a dramatic increase  of Tg binding to BiP and GRP94.	bind
11625	2	4579	5	NULL	NULL	0	NULL	CST	NULL		increase	NULL	dramatically			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_22_9793_s_263	16260597	(C) CST causes a dramatic increase  of Tg binding to BiP and GRP94.	bind
11626	3	4579	5	NULL	NULL	0	NULL	Tg	NULL		bind	NULL				GRP94	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_22_9793_s_263	16260597	(C) CST causes a dramatic increase  of Tg binding to BiP and GRP94.	bind
11627	4	4579	5	NULL	NULL	0	NULL	CST	NULL		increase	NULL	dramatically			statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_22_9793_s_263	16260597	(C) CST causes a dramatic increase  of Tg binding to BiP and GRP94.	bind
11578	1	4579	6	NULL	NULL	NULL	NULL	Tg	GP		bind					BiP	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9793_s_263	16260597	(C) CST causes a dramatic increase  of Tg binding to BiP and GRP94.	bind
11579	2	4579	6	NULL	NULL	NULL	NULL	Tg	GP		bind					GRP94	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9793_s_263	16260597	(C) CST causes a dramatic increase  of Tg binding to BiP and GRP94.	bind
11580	3	4579	6	NULL	NULL	NULL	NULL	CST	GP		increases		dramatically			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9793_s_263	16260597	(C) CST causes a dramatic increase  of Tg binding to BiP and GRP94.	bind
11581	4	4579	6	NULL	NULL	NULL	NULL	CST	GP		increases		dramatically			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9793_s_263	16260597	(C) CST causes a dramatic increase  of Tg binding to BiP and GRP94.	bind
11628	1	4580	5	NULL	NULL	0	NULL	CTGF	NULL		bind	NULL				LRP6	NULL		EGF repeat 1		NULL		0	NULL	NULL	NULL	gw70_development_131_9_2137_s_237	15105373	(C) CTGF binds to both EGF repeats 1, 2 and 3, 4 of LRP6.	bind
11629	2	4580	5	NULL	NULL	0	NULL	CTGF	NULL		bind	NULL				LRP6	NULL		EGF repeat 2		NULL		0	NULL	NULL	NULL	gw70_development_131_9_2137_s_237	15105373	(C) CTGF binds to both EGF repeats 1, 2 and 3, 4 of LRP6.	bind
11630	3	4580	5	NULL	NULL	0	NULL	CTGF	NULL		bind	NULL				LRP6	NULL		EGF repeat 3		NULL		0	NULL	NULL	NULL	gw70_development_131_9_2137_s_237	15105373	(C) CTGF binds to both EGF repeats 1, 2 and 3, 4 of LRP6.	bind
11631	4	4580	5	NULL	NULL	0	NULL	CTGF	NULL		bind	NULL				LRP6	NULL		EGF repeat 4		NULL		0	NULL	NULL	NULL	gw70_development_131_9_2137_s_237	15105373	(C) CTGF binds to both EGF repeats 1, 2 and 3, 4 of LRP6.	bind
11582	1	4580	6	NULL	NULL	NULL	NULL	CTGF	GP		bind					LRP6	GP		EGF repeat 1		NULL		NULL	NULL	NULL	NULL	gw70_development_131_9_2137_s_237	15105373	(C) CTGF binds to both EGF repeats 1, 2 and 3, 4 of LRP6.	bind
13007	2	4580	6	NULL	NULL	NULL	NULL	CTGF	GP		bind					LRP6	GP		EGF repeat 2		NULL		NULL	NULL	NULL	NULL	gw70_development_131_9_2137_s_237	15105373	(C) CTGF binds to both EGF repeats 1, 2 and 3, 4 of LRP6.	bind
13008	3	4580	6	NULL	NULL	NULL	NULL	CTGF	GP		bind					LRP6	GP		EGF repeat 3		NULL		NULL	NULL	NULL	NULL	gw70_development_131_9_2137_s_237	15105373	(C) CTGF binds to both EGF repeats 1, 2 and 3, 4 of LRP6.	bind
13009	4	4580	6	NULL	NULL	NULL	NULL	CTGF	GP		bind					LRP6	GP		EGF repeat 4		NULL		NULL	NULL	NULL	NULL	gw70_development_131_9_2137_s_237	15105373	(C) CTGF binds to both EGF repeats 1, 2 and 3, 4 of LRP6.	bind
11632	1	4581	5	NULL	NULL	0	NULL	Cux/CDP	NULL		bind	NULL					NULL			P1 site	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_1_284_s_182	9858552	(C) Cux/CDP binds to P1, P2, and P4 sites.	bind
11633	2	4581	5	NULL	NULL	0	NULL	Cux/CDP	NULL		bind	NULL					NULL			P2 site	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_1_284_s_182	9858552	(C) Cux/CDP binds to P1, P2, and P4 sites.	bind
11634	3	4581	5	NULL	NULL	0	NULL	Cux/CDP	NULL		bind	NULL					NULL			P4 site	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_1_284_s_182	9858552	(C) Cux/CDP binds to P1, P2, and P4 sites.	bind
11583	1	4581	6	NULL	NULL	NULL	NULL	Cux/CDP	GP		bind									P1 site	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_284_s_182	9858552	(C) Cux/CDP binds to P1, P2, and P4 sites.	bind
11584	2	4581	6	NULL	NULL	NULL	NULL	Cux/CDP	GP		bind									P2 site	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_284_s_182	9858552	(C) Cux/CDP binds to P1, P2, and P4 sites.	bind
11585	3	4581	6	NULL	NULL	NULL	NULL	Cux/CDP	GP		bind									P4 site	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_284_s_182	9858552	(C) Cux/CDP binds to P1, P2, and P4 sites.	bind
11635	1	4582	5	NULL	NULL	0	NULL	Cyclin E	NULL	alone	does not bind	NULL				p300	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_136	10330164	(C) Cyclin E alone does not bind to p300.	bind
11586	1	4582	6	NULL	NULL	NULL	NULL	Cyclin E	GP		does not bind					p300	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_136	10330164	(C) Cyclin E alone does not bind to p300.	bind
11636	1	4583	5	NULL	NULL	0	NULL	Sir3	NULL		bind	NULL				Sir4	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_11_4514_s_199	15899856	(C) Defects in Sir3 binding to Sir4 derepress telomeric silencing.	bind
11637	2	4583	5	NULL	NULL	0	NULL	statement 1	NULL	defects in	derepress	NULL				telomeric silencing	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_11_4514_s_199	15899856	(C) Defects in Sir3 binding to Sir4 derepress telomeric silencing.	bind
11587	1	4583	6	NULL	NULL	NULL	NULL	Sir3	GP		bind					Sir4	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_11_4514_s_199	15899856	(C) Defects in Sir3 binding to Sir4 derepress telomeric silencing.	bind
11588	2	4583	6	NULL	NULL	NULL	NULL	statement 1	Process	defects in	derepress					telomeric silencing	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_11_4514_s_199	15899856	(C) Defects in Sir3 binding to Sir4 derepress telomeric silencing.	bind
11638	1	4584	5	NULL	NULL	0	NULL	mGluR7a	NULL		bind	NULL				PICK1	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_28_2_485_s_47	11144358	(C) Deletion of last 3 amino acids of the distal tail of mGluR7a (distal 7a 3) eliminated the binding with PICK1.	bind
11639	2	4584	5	NULL	NULL	0	NULL		NULL		eliminate	NULL		distal 7a 3		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuron_28_2_485_s_47	11144358	(C) Deletion of last 3 amino acids of the distal tail of mGluR7a (distal 7a 3) eliminated the binding with PICK1.	bind
11640	3	4584	5	NULL	NULL	0	NULL	distal 7a 3	NULL		is	NULL				deletion of last 3 amino acids of the distal tail of mGluR7a	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_28_2_485_s_47	11144358	(C) Deletion of last 3 amino acids of the distal tail of mGluR7a (distal 7a 3) eliminated the binding with PICK1.	bind
11589	1	4584	6	NULL	NULL	NULL	NULL	mGluR7a	GP		bind					PICK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_28_2_485_s_47	11144358	(C) Deletion of last 3 amino acids of the distal tail of mGluR7a (distal 7a 3) eliminated the binding with PICK1.	bind
11590	2	4584	6	NULL	NULL	NULL	NULL	mGluR7a	GP	deletion mutant	eliminates			distal 7a 3		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_28_2_485_s_47	11144358	(C) Deletion of last 3 amino acids of the distal tail of mGluR7a (distal 7a 3) eliminated the binding with PICK1.	bind
13010	3	4584	6	NULL	NULL	NULL	NULL	distal 7a			is					deletion of last 3 amino acids of the distal tail of mGluR7a					NULL		NULL	NULL	NULL	NULL	gw60_neuron_28_2_485_s_47	11144358	(C) Deletion of last 3 amino acids of the distal tail of mGluR7a (distal 7a 3) eliminated the binding with PICK1.	bind
11641	1	4585	5	NULL	NULL	0	NULL	paxillin	NULL		bind	NULL		NH2 terminus		p95PKL	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_4_851_s_269	10330411	(C) Deletion of LD4 from the paxillin NH2 terminus fusion protein eliminated the binding to p95PKL.	bind
11642	2	4585	5	NULL	NULL	0	NULL	paxillin	NULL	deletion of LD4 from	eliminate	NULL		NH2 terminus		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_4_851_s_269	10330411	(C) Deletion of LD4 from the paxillin NH2 terminus fusion protein eliminated the binding to p95PKL.	bind
44563	3	4585	5	10	NULL	0	NULL	paxillin	NULL		is a type of	NULL				fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_4_851_s_269	10330411	(C) Deletion of LD4 from the paxillin NH2 terminus fusion protein eliminated the binding to p95PKL.	bind
11591	1	4585	6	NULL	NULL	NULL	NULL	paxillin	GP		bind			NH2 terminus		p95PKL	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_4_851_s_269	10330411	(C) Deletion of LD4 from the paxillin NH2 terminus fusion protein eliminated the binding to p95PKL.	bind
11592	2	4585	6	NULL	NULL	NULL	NULL	paxillin 	GP	deletion of LD4 from	eliminates			NH2 terminus		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_4_851_s_269	10330411	(C) Deletion of LD4 from the paxillin NH2 terminus fusion protein eliminated the binding to p95PKL.	bind
54441	3	4585	6	NULL	NULL	NULL	NULL	 paxillin	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_4_851_s_269	10330411	(C) Deletion of LD4 from the paxillin NH2 terminus fusion protein eliminated the binding to p95PKL.	bind
11644	1	4589	5	NULL	NULL	0	NULL	JIP-1	NULL		bind	NULL	differentially			APP polypeptides	NULL	phosphorylated			NULL		0	NULL	NULL	NULL	gw70_cellbiol_171_4_615_s_92	16301330	(C) Differential  binding of JIP-1 and Fe65 to phosphorylated and nonphosphorylated APP polypeptides  (ELISA).	bind
11645	2	4589	5	NULL	NULL	0	NULL	JIP-1	NULL		bind	NULL	differentially			APP polypeptides	NULL	nonphosphorylated			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_4_615_s_92	16301330	(C) Differential  binding of JIP-1 and Fe65 to phosphorylated and nonphosphorylated APP polypeptides  (ELISA).	bind
11646	3	4589	5	NULL	NULL	0	NULL	Fe65	NULL		bind	NULL	differentially			APP polypeptides	NULL	phosphorylated			NULL		0	NULL	NULL	NULL	gw70_cellbiol_171_4_615_s_92	16301330	(C) Differential  binding of JIP-1 and Fe65 to phosphorylated and nonphosphorylated APP polypeptides  (ELISA).	bind
11647	4	4589	5	NULL	NULL	0	NULL	Fe65	NULL		bind	NULL	differentially			APP polypeptides	NULL	nonphosphorylated			NULL		0	NULL	NULL	NULL	gw70_cellbiol_171_4_615_s_92	16301330	(C) Differential  binding of JIP-1 and Fe65 to phosphorylated and nonphosphorylated APP polypeptides  (ELISA).	bind
11593	1	4589	6	NULL	NULL	NULL	NULL	JIP1	GP		bind		differentially			APP polypeptides	AminoAcid	phosphorylated			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_4_615_s_92	16301330	(C) Differential  binding of JIP-1 and Fe65 to phosphorylated and nonphosphorylated APP polypeptides  (ELISA).	bind
11594	2	4589	6	NULL	NULL	NULL	NULL	JIP1	GP		bind		differentially			APP polypeptides	AminoAcid	nonphosphorylated			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_4_615_s_92	16301330	(C) Differential  binding of JIP-1 and Fe65 to phosphorylated and nonphosphorylated APP polypeptides  (ELISA).	bind
11595	3	4589	6	NULL	NULL	NULL	NULL	Fe65	GP		bind		differentially			APP polypeptides	AminoAcid	phosphorylated			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_4_615_s_92	16301330	(C) Differential  binding of JIP-1 and Fe65 to phosphorylated and nonphosphorylated APP polypeptides  (ELISA).	bind
11596	4	4589	6	NULL	NULL	NULL	NULL	Fe65	GP		bind		differentially			APP polypeptides	AminoAcid	nonphosphorylated			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_4_615_s_92	16301330	(C) Differential  binding of JIP-1 and Fe65 to phosphorylated and nonphosphorylated APP polypeptides  (ELISA).	bind
11648	1	4590	5	NULL	NULL	0	NULL	s-synaphin constructs	NULL	recombinant	bind	NULL	differentially			syntaxin	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_104_3_421_s_58	11239399	(C) Differential binding of recombinant s-synaphin constructs to syntaxin.	bind
11597	1	4590	6	NULL	NULL	NULL	NULL	s-synaphin	GP	recombinant	bind		differentially			syntaxin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_104_3_421_s_58	11239399	(C) Differential binding of recombinant s-synaphin constructs to syntaxin.	bind
11658	1	4591	5	NULL	NULL	0	NULL	TCF	NULL		bind	NULL				beta-catenin	NULL	untethered 			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8462_s_163	14612392	(C) Differential requirements of TCF and APC binding for untethered  and membrane-tethered beta-catenin.	bind
11659	2	4591	5	NULL	NULL	0	NULL	APC	NULL		bind	NULL				beta-catenin	NULL	untethered			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8462_s_163	14612392	(C) Differential requirements of TCF and APC binding for untethered  and membrane-tethered beta-catenin.	bind
11660	3	4591	5	NULL	NULL	0	NULL	TCF	NULL		bind	NULL				beta-catenin	NULL	membrane-tethered			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8462_s_163	14612392	(C) Differential requirements of TCF and APC binding for untethered  and membrane-tethered beta-catenin.	bind
11661	4	4591	5	NULL	NULL	0	NULL	APC	NULL		bind	NULL				beta-catenin	NULL	membrane-tethered			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8462_s_163	14612392	(C) Differential requirements of TCF and APC binding for untethered  and membrane-tethered beta-catenin.	bind
43796	1	4591	6	NULL	NULL	NULL	NULL	beta-catenin	GP	untethered	bind					TCF	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8462_s_163	14612392	(C) Differential requirements of TCF and APC binding for untethered  and membrane-tethered beta-catenin.	bind
43797	2	4591	6	NULL	NULL	NULL	NULL	beta-catenin	GP	membrane-tethered	bind					TCF	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8462_s_163	14612392	(C) Differential requirements of TCF and APC binding for untethered  and membrane-tethered beta-catenin.	bind
43798	3	4591	6	NULL	NULL	NULL	NULL	beta-catenin	GP	untethered	bind					APC	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8462_s_163	14612392	(C) Differential requirements of TCF and APC binding for untethered  and membrane-tethered beta-catenin.	bind
43799	4	4591	6	NULL	NULL	NULL	NULL	beta-catenin	GP	membrane-tethered	bind					APC	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8462_s_163	14612392	(C) Differential requirements of TCF and APC binding for untethered  and membrane-tethered beta-catenin.	bind
11656	1	4592	5	10	NULL	0	NULL	DDR1 Rbodies			bind		differentially			dermal collagen I		 bovine			NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_131	9659900	(C) Differential slot-blot binding of DDR1 and DDR2 Rbodies to commercially-derived bovine dermal collagen I (Vitrogen).	bind
11657	2	4592	5	10	NULL	0	NULL	DDR2 Rbodies			bind		differentially			dermal collagen I		 bovine			NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_131	9659900	(C) Differential slot-blot binding of DDR1 and DDR2 Rbodies to commercially-derived bovine dermal collagen I (Vitrogen).	bind
11674	1	4592	6	NULL	NULL	NULL	NULL	DDR1 Rbodies	GP		bind		differentially			dermal collagen I	GP	bovine			NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_131	9659900	(C) Differential slot-blot binding of DDR1 and DDR2 Rbodies to commercially-derived bovine dermal collagen I (Vitrogen).	bind
11675	2	4592	6	NULL	NULL	NULL	NULL	DDR2 Rbodies	GP		bind		differentially			dermal collagen I	GP	bovine			NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_1_25_s_131	9659900	(C) Differential slot-blot binding of DDR1 and DDR2 Rbodies to commercially-derived bovine dermal collagen I (Vitrogen).	bind
11662	1	4593	5	NULL	NULL	0	NULL	GST-p53	NULL	recombinant	bind	NULL	directly				NULL			 p53BE	NULL		NULL	NULL	NULL	NULL	gw60_cell_113_3_301_s_280	12732139	(C) Direct binding of recombinant GST-p53 and p73 to the  p53BE in gel shift experiments.	bind
11664	2	4593	5	NULL	NULL	0	NULL	GST-p73	NULL	recombinant	bind	NULL	directly				NULL			p53BE	NULL		NULL	NULL	NULL	NULL	gw60_cell_113_3_301_s_280	12732139	(C) Direct binding of recombinant GST-p53 and p73 to the  p53BE in gel shift experiments.	bind
11676	1	4593	6	NULL	NULL	NULL	NULL	GST-p53	GP	recombinant	bind		directly							p53BE	NULL		NULL	NULL	NULL	NULL	gw60_cell_113_3_301_s_280	12732139	(C) Direct binding of recombinant GST-p53 and p73 to the  p53BE in gel shift experiments.	bind
11677	2	4593	6	NULL	NULL	NULL	NULL	GST-p73	GP	recombinant	bind		directly							p53BE	NULL		NULL	NULL	NULL	NULL	gw60_cell_113_3_301_s_280	12732139	(C) Direct binding of recombinant GST-p53 and p73 to the  p53BE in gel shift experiments.	bind
11665	1	4594	5	NULL	NULL	0	NULL	Stx6	NULL		bind	NULL	directly			Syt IV	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw70_cellbiol_173_2_241_s_130	16618809	(C) Direct binding of Stx6  to Syt IV in vitro.	bind
11678	1	4594	6	NULL	NULL	NULL	NULL	Stx6	GP		bind		directly			Syt IV	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_cellbiol_173_2_241_s_130	16618809	(C) Direct binding of Stx6  to Syt IV in vitro.	bind
11666	1	4596	5	NULL	NULL	0	NULL	[125]AFP	NULL		bind	NULL				MDM	NULL				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_3_507_s_104	12176010	(C) Displacement curve shows inhibition of the binding of [125]AFP (1.5 nM) to MDM by unlabeled AFP.	bind
11667	2	4596	5	NULL	NULL	0	NULL	AFP	NULL	unlabeled	inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_3_507_s_104	12176010	(C) Displacement curve shows inhibition of the binding of [125]AFP (1.5 nM) to MDM by unlabeled AFP.	bind
11679	1	4596	6	NULL	NULL	NULL	NULL	[125]AFP	Chemical		bind					MDM	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_3_507_s_104	12176010	(C) Displacement curve shows inhibition of the binding of [125]AFP (1.5 nM) to MDM by unlabeled AFP.	bind
11680	2	4596	6	NULL	NULL	NULL	NULL	AFP	Chemical	unlabeled	inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_3_507_s_104	12176010	(C) Displacement curve shows inhibition of the binding of [125]AFP (1.5 nM) to MDM by unlabeled AFP.	bind
11668	1	4597	5	10	NULL	0	NULL	RFX			bind					DRA				promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_17_5699_s_350	11486010	(C) Dissociation rates were determined by EMSA for the higher-order protein-DNA complexes formed by simultaneous binding of RFX, NF-Y, and X2BP to the DRA promoter.	bind
11669	2	4597	5	NULL	NULL	0	NULL	NF-Y	NULL		bind	NULL				DRA	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_17_5699_s_350	11486010	(C) Dissociation rates were determined by EMSA for the higher-order protein-DNA complexes formed by simultaneous binding of RFX, NF-Y, and X2BP to the DRA promoter.	bind
11670	3	4597	5	NULL	NULL	0	NULL	X2BP	NULL		bind	NULL				DRA	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_17_5699_s_350	11486010	(C) Dissociation rates were determined by EMSA for the higher-order protein-DNA complexes formed by simultaneous binding of RFX, NF-Y, and X2BP to the DRA promoter.	bind
11681	1	4597	6	NULL	NULL	NULL	NULL	RFX	GP		bind					DRA	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_17_5699_s_350	11486010	(C) Dissociation rates were determined by EMSA for the higher-order protein-DNA complexes formed by simultaneous binding of RFX, NF-Y, and X2BP to the DRA promoter.	bind
11682	2	4597	6	NULL	NULL	NULL	NULL	NF-Y	GP		bind					DRA	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_17_5699_s_350	11486010	(C) Dissociation rates were determined by EMSA for the higher-order protein-DNA complexes formed by simultaneous binding of RFX, NF-Y, and X2BP to the DRA promoter.	bind
11683	3	4597	6	NULL	NULL	NULL	NULL	X2BP	GP		bind					DRA	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_17_5699_s_350	11486010	(C) Dissociation rates were determined by EMSA for the higher-order protein-DNA complexes formed by simultaneous binding of RFX, NF-Y, and X2BP to the DRA promoter.	bind
11671	1	4599	5	NULL	NULL	0	NULL	Dll3	NULL	expression of	is restricted to	NULL				Purkinje cells	NULL				NULL	adult cerebellum	0	NULL	NULL	NULL	gw60_mechdev_114_1_153_s_128	12175503	(C) Dll3 expression is restricted to Purkinje cells (PC; arrow) in the adult cerebellum and, (D) Jagged1 is prominently expressed by granule cells in the IGL.	bind
11672	2	4599	5	10	NULL	0	NULL	Jagged1			is expressed by		prominently			granule cells					NULL	IGL	NULL	NULL	NULL	NULL	gw60_mechdev_114_1_153_s_128	12175503	(C) Dll3 expression is restricted to Purkinje cells (PC; arrow) in the adult cerebellum and, (D) Jagged1 is prominently expressed by granule cells in the IGL.	bind
11684	1	4599	6	NULL	NULL	NULL	NULL	Purkinje cells	Cell		express					dll3	GP				NULL	adult cerebellum	NULL	NULL	NULL	NULL	gw60_mechdev_114_1_153_s_128	12175503	(C) Dll3 expression is restricted to Purkinje cells (PC; arrow) in the adult cerebellum and, (D) Jagged1 is prominently expressed by granule cells in the IGL.	bind
11685	2	4599	6	NULL	NULL	NULL	NULL	granule cells	Cell		express					Jagged1	GP				NULL	IGL	NULL	NULL	NULL	NULL	gw60_mechdev_114_1_153_s_128	12175503	(C) Dll3 expression is restricted to Purkinje cells (PC; arrow) in the adult cerebellum and, (D) Jagged1 is prominently expressed by granule cells in the IGL.	bind
11673	1	4600	5	10	NULL	0	NULL	PerR	NULL	purified	bind	NULL				perR	NULL			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_12_3276_s_146	12029044	(C) DNase I footprint of purified PerR binding to the  perR promoter.	bind
11686	1	4600	6	NULL	NULL	NULL	NULL	PerR	GP	purified	bind					perR	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_12_3276_s_146	12029044	(C) DNase I footprint of purified PerR binding to the  perR promoter.	bind
11933	1	4601	5	NULL	NULL	0	NULL	Dock	NULL		bind	NULL	directly	SH2		Dscam	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cell_101_6_671_s_111	10892653	(C) Dock SH2  directly binds Dscam.	bind
11687	1	4601	6	NULL	NULL	NULL	NULL	Dock	GP		bind		directly	SH2 domain		Dscam	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_101_6_671_s_111	10892653	(C) Dock SH2  directly binds Dscam.	bind
11934	1	4602	5	NULL	NULL	0	NULL	DOKL	NULL		bind	NULL				c-Abl	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_12_8314_s_280	10567556	(C) DOKL binding to c-Abl can be detected with anti-Abl antisera.	bind
11688	1	4602	6	NULL	NULL	NULL	NULL	DOKL	GP		bind					c-Abl	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8314_s_280	10567556	(C) DOKL binding to c-Abl can be detected with anti-Abl antisera.	bind
12084	2	4603	5	NULL	NULL	0	NULL	SfbX	NULL	recombinant	bind	NULL				fibronectin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_4_1208_s_215	12562790	(c) Dose-dependent competitive inhibition of GAS fibronectin-binding by recombinant SfbX.	bind
14577	3	4603	5	10	NULL	0	NULL	statement 2	NULL		inhibit	NULL	competitively;;dose dependently			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_4_1208_s_215	12562790	(c) Dose-dependent competitive inhibition of GAS fibronectin-binding by recombinant SfbX.	bind
14578	1	4603	5	NULL	NULL	0	NULL	GAS	NULL		bind	NULL				fibronectin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_185_4_1208_s_215	12562790	(c) Dose-dependent competitive inhibition of GAS fibronectin-binding by recombinant SfbX.	bind
11689	1	4603	6	NULL	NULL	NULL	NULL	GAS	GP		bind					fibronectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_4_1208_s_215	12562790	(c) Dose-dependent competitive inhibition of GAS fibronectin-binding by recombinant SfbX.	bind
11690	2	4603	6	NULL	NULL	NULL	NULL	Sfbx	GP	recombinant	bind					fibronectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_4_1208_s_215	12562790	(c) Dose-dependent competitive inhibition of GAS fibronectin-binding by recombinant SfbX.	bind
11691	3	4603	6	NULL	NULL	NULL	NULL	statement 2	Process		inhibits		competitively;;dose dependently			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_4_1208_s_215	12562790	(c) Dose-dependent competitive inhibition of GAS fibronectin-binding by recombinant SfbX.	bind
12086	1	4604	5	10	NULL	0	NULL	Ndc10p			bind					Chromosome V					NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_11_4557_s_180	13679521	(C) Doubling time under nonselective conditions (YPD); chromosome  loss rates determined from B. (D) Binding of Ndc10p and the cohesin subunit Mcd1p  to a region of Chromosome V previously subjected to detailed analysis (Tanaka  et al., 1999 ) by ChIP in 200-base pair DNA fragments spaced every 1 kb.	bind
12088	2	4604	5	10	NULL	0	NULL	Mcd1p			bind			cohesin subunit		Chromosome V					NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_11_4557_s_180	13679521	(C) Doubling time under nonselective conditions (YPD); chromosome  loss rates determined from B. (D) Binding of Ndc10p and the cohesin subunit Mcd1p  to a region of Chromosome V previously subjected to detailed analysis (Tanaka  et al., 1999 ) by ChIP in 200-base pair DNA fragments spaced every 1 kb.	bind
11692	1	4604	6	NULL	NULL	NULL	NULL	Ndc10p	GP		bind					region of Chromosome V	Chromosome				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_11_4557_s_180	13679521	(C) Doubling time under nonselective conditions (YPD); chromosome  loss rates determined from B. (D) Binding of Ndc10p and the cohesin subunit Mcd1p  to a region of Chromosome V previously subjected to detailed analysis (Tanaka  et al., 1999 ) by ChIP in 200-base pair DNA fragments spaced every 1 kb.	bind
11693	2	4604	6	NULL	NULL	NULL	NULL	Mcd1p	GP		bind			cohesin subunit		region of Chromosome V	Chromosome				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_11_4557_s_180	13679521	(C) Doubling time under nonselective conditions (YPD); chromosome  loss rates determined from B. (D) Binding of Ndc10p and the cohesin subunit Mcd1p  to a region of Chromosome V previously subjected to detailed analysis (Tanaka  et al., 1999 ) by ChIP in 200-base pair DNA fragments spaced every 1 kb.	bind
12090	1	4605	5	NULL	NULL	0	NULL	RFP - X-PAK5	NULL		bind	NULL				GFP MT bundles	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_155_6_1029_s_214	11733543	(C) Dynamic of RFP - X-PAK5 - bound GFP MT bundles (the dot pinpoints the initial position of the free end of a bundle) versus unbound GFP MTs (the cross pinpoints the initial position of one MT) were overlaid.	bind
11694	1	4605	6	NULL	NULL	NULL	NULL	RFP - X-PAK5	GP		bind					GFP MT bundles	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_1029_s_214	11733543	(C) Dynamic of RFP - X-PAK5 - bound GFP MT bundles (the dot pinpoints the initial position of the free end of a bundle) versus unbound GFP MTs (the cross pinpoints the initial position of one MT) were overlaid.	bind
12098	1	4606	5	NULL	NULL	0	NULL	Rb	NULL		inhibit	NULL				E2F	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_18_6799_s_117	10958676	(C) E1a cannot block Rb inhibition of E2F when the LXCXE binding site is mutated.	bind
12105	2	4606	5	NULL	NULL	0	NULL	E1a	NULL	mutant	does not block	NULL		LXCXE binding site		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_18_6799_s_117	10958676	(C) E1a cannot block Rb inhibition of E2F when the LXCXE binding site is mutated.	bind
12187	3	4606	5	NULL	NULL	0	NULL	E1a	NULL		blocks	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_18_6799_s_117	10958676	(C) E1a cannot block Rb inhibition of E2F when the LXCXE binding site is mutated.	bind
12301	1	4606	6	NULL	NULL	NULL	NULL	Rb	GP		inhibits					E2F	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_18_6799_s_117	10958676	(C) E1a cannot block Rb inhibition of E2F when the LXCXE binding site is mutated.	bind
12302	2	4606	6	NULL	NULL	NULL	NULL	E1a	GP		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_18_6799_s_117	10958676	(C) E1a cannot block Rb inhibition of E2F when the LXCXE binding site is mutated.	bind
12303	3	4606	6	NULL	NULL	NULL	NULL	E1a	GP	mutant	does not block			LXCXE binding site		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_18_6799_s_117	10958676	(C) E1a cannot block Rb inhibition of E2F when the LXCXE binding site is mutated.	bind
12108	1	4607	5	NULL	NULL	0	NULL	E1B 55-kDa proteins	NULL		bind	NULL				PCAF	NULL				NULL	in vivo	0	NULL	NULL	NULL	gw60_molcellbiol_20_15_5540_s_306	10891493	(C) E1B 55-kDa proteins bind to PCAF in vivo.	bind
11695	1	4607	6	NULL	NULL	NULL	NULL	E1B 55-kDa proteins	GP		bind					PCAF	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5540_s_306	10891493	(C) E1B 55-kDa proteins bind to PCAF in vivo.	bind
12138	1	4608	5	NULL	NULL	0	NULL	EBNA-1	NULL		bind	NULL		delta16-372		oriP plasmids	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_10_3576_s_222	11313483	(C) EBNA-1(delta16-372) can bind  oriP plasmids but cannot recruit them onto mitotic chromosomes.	bind
12141	3	4608	5	NULL	NULL	0	NULL	EBNA-1	NULL		does not recruit	NULL		delta16-372		statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_10_3576_s_222	11313483	(C) EBNA-1(delta16-372) can bind  oriP plasmids but cannot recruit them onto mitotic chromosomes.	bind
44564	2	4608	5	10	NULL	0	NULL	oriP	NULL		recruits to	NULL				mitotic chromosomes	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_10_3576_s_222	11313483	(C) EBNA-1(delta16-372) can bind  oriP plasmids but cannot recruit them onto mitotic chromosomes.	bind
11696	1	4608	6	NULL	NULL	NULL	NULL	EBNA-1	GP		bind			delta16-372		oriP plasmids	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_10_3576_s_222	11313483	(C) EBNA-1(delta16-372) can bind  oriP plasmids but cannot recruit them onto mitotic chromosomes.	bind
54450	2	4608	6	NULL	NULL	NULL	NULL	oriP	NucleicAcid		recruits to					mitotic chromosomes	Chromosome				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_10_3576_s_222	11313483	(C) EBNA-1(delta16-372) can bind  oriP plasmids but cannot recruit them onto mitotic chromosomes.	bind
54451	3	4608	6	NULL	NULL	NULL	NULL	EBNA-1	GP		does not recruit			delta16-372		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_10_3576_s_222	11313483	(C) EBNA-1(delta16-372) can bind  oriP plasmids but cannot recruit them onto mitotic chromosomes.	bind
12144	1	4610	5	NULL	NULL	0	NULL	Npl3p	NULL		bind	NULL				Mtr10p	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_150_4_707_s_209	10952997	(c) Effect of double modification on Npl3p binding to Mtr10p.	bind
11697	1	4610	6	NULL	NULL	NULL	NULL	Npl3p	GP		bind					Mtr10p	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_150_4_707_s_209	10952997	(c) Effect of double modification on Npl3p binding to Mtr10p.	bind
12148	1	4611	5	NULL	NULL	0	NULL	LARG	NULL		bind	NULL				IGF-1 receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_155_5_809_s_122	11724822	(C) Effect of IGF-1 on the binding state of LARG and the IGF-1 receptor.	bind
11698	1	4611	6	NULL	NULL	NULL	NULL	LARG	GP		bind					IGF-1 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_5_809_s_122	11724822	(C) Effect of IGF-1 on the binding state of LARG and the IGF-1 receptor.	bind
12167	1	4612	5	NULL	NULL	0	NULL	sAPP695T	NULL		bind	NULL				HK	NULL	cleavage products of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1571_3_225_s_253	12090937	(C) Effect of plasma kallikrein treatment on binding of sAPP695T to HK cleavage products.	bind
11699	1	4612	6	NULL	NULL	NULL	NULL	sAPP695T			bind					HK 	GP	clevage products of			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1571_3_225_s_253	12090937	(C) Effect of plasma kallikrein treatment on binding of sAPP695T to HK cleavage products.	bind
12168	1	4614	5	NULL	NULL	0	NULL	fascin	NULL		bind	NULL				actin	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_150_4_807_s_276	10953005	(C) Effect of the antibodies on the binding of fascin to actin in a blot-overlay assay.	bind
11700	1	4614	6	NULL	NULL	NULL	NULL	fascin	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_150_4_807_s_276	10953005	(C) Effect of the antibodies on the binding of fascin to actin in a blot-overlay assay.	bind
12169	1	4615	5	NULL	NULL	0	NULL	A1Rs	NULL		bind	NULL				hsc73	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_14_5164_s_206	10866672	(C) Effect of two different concentrations of ADA upon binding of A1Rs to hsc73.	bind
11701	1	4615	6	NULL	NULL	NULL	NULL	A1Rs	GP		bind					hsc73	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_14_5164_s_206	10866672	(C) Effect of two different concentrations of ADA upon binding of A1Rs to hsc73.	bind
12170	1	4616	5	NULL	NULL	0	NULL	IAAP	NULL		bind	NULL				Cdr1p-GFP	NULL				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_2_6_1361_s_192	14665469	(c) Effects of Cdr1p substrates on the binding of IAAP to  Cdr1p-GFP.	bind
11702	1	4616	6	NULL	NULL	NULL	NULL	IAAP	GP		bind					Cdr1p-GFP	GP				NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_2_6_1361_s_192	14665469	(c) Effects of Cdr1p substrates on the binding of IAAP to  Cdr1p-GFP.	bind
12171	1	4617	5	NULL	NULL	0	NULL	BMP-7	NULL		bind	NULL				ROS 17/2	NULL				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_308_4_858_s_198	12927798	(C) Effects of GAGs on BMP-7 binding to ROS 17/2.	bind
11703	1	4617	6	NULL	NULL	NULL	NULL	BMP-7	GP		bind					ROS 17/2	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_308_4_858_s_198	12927798	(C) Effects of GAGs on BMP-7 binding to ROS 17/2.	bind
12172	1	4618	5	NULL	NULL	0	NULL	LDL	NULL		bind	NULL				CHO-CD36 cells	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_40_4_753_s_117	10191300	(C) Effects of peptide V on the binding of LDL to CHO-CD36 cells.	bind
11704	1	4618	6	NULL	NULL	NULL	NULL	LDL	Chemical		bind					CHO-CD36 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_4_753_s_117	10191300	(C) Effects of peptide V on the binding of LDL to CHO-CD36 cells.	bind
12188	1	4619	5	NULL	NULL	0	NULL	Axn follicle cell clones	NULL	mutant	express	NULL				Hts	NULL	higher levels of			NULL	Egg chambers	0	NULL	NULL	NULL	gw60_development_130_14_3259_s_211	12783796	(C) Egg chambers with mutant  Axn follicle cell clones that express higher levels of Hts (outlined).	bind
11705	1	4619	6	NULL	NULL	NULL	NULL	 Axn follicle cell clones	Cell	mutant	express					Hts	GP	high levels of			NULL	Egg chambers	NULL	NULL	NULL	NULL	gw60_development_130_14_3259_s_211	12783796	(C) Egg chambers with mutant  Axn follicle cell clones that express higher levels of Hts (outlined).	bind
12189	1	4620	5	NULL	NULL	0	NULL	Elc1	NULL		bind	NULL				Snf4	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1491_1_161_s_309	10760578	(C) Elc1 binding to Snf4 is not for required for glucose derepression.	bind
12190	2	4620	5	NULL	NULL	0	NULL	statement 1	NULL		is not required for	NULL				glucose derepression	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1491_1_161_s_309	10760578	(C) Elc1 binding to Snf4 is not for required for glucose derepression.	bind
11706	1	4620	6	NULL	NULL	NULL	NULL	Elc1	GP		bind					Snf4	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1491_1_161_s_309	10760578	(C) Elc1 binding to Snf4 is not for required for glucose derepression.	bind
11707	2	4620	6	NULL	NULL	NULL	NULL	statement 1	Process		is not required for					glucose derepression	AbstractConcept				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1491_1_161_s_309	10760578	(C) Elc1 binding to Snf4 is not for required for glucose derepression.	bind
12191	1	4625	5	NULL	NULL	0	NULL	AlgR	NULL		bind	NULL				algD sequences	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_16_4544_s_181	12142425	(C) EMSA of AlgR or AlgR derivatives binding to  algD sequences.	bind
12192	2	4625	5	NULL	NULL	0	NULL	AlgR derivatives	NULL		bind	NULL				algD sequences	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_16_4544_s_181	12142425	(C) EMSA of AlgR or AlgR derivatives binding to  algD sequences.	bind
12194	3	4625	5	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_16_4544_s_181	12142425	(C) EMSA of AlgR or AlgR derivatives binding to  algD sequences.	bind
11708	1	4625	6	NULL	NULL	NULL	NULL	AlgR	GP		bind					algD sequences	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_16_4544_s_181	12142425	(C) EMSA of AlgR or AlgR derivatives binding to  algD sequences.	bind
11709	2	4625	6	NULL	NULL	NULL	NULL	AlgR derivatives 	GP		bind					algD sequences	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_16_4544_s_181	12142425	(C) EMSA of AlgR or AlgR derivatives binding to  algD sequences.	bind
11710	3	4625	6	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_16_4544_s_181	12142425	(C) EMSA of AlgR or AlgR derivatives binding to  algD sequences.	bind
12193	1	4627	5	NULL	NULL	0	NULL	c- myc RNA	NULL		does not bind	NULL			IRES	unr	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_10_3364_s_143	11313462	(C) EMSA of c- myc IRES RNA does not show any binding to unr or PTB. (D) EMSA of G3PDH mRNA used a control does not show any binding to unr or PTB.	bind
12195	2	4627	5	NULL	NULL	0	NULL	c- myc RNA	NULL		does not bind	NULL			IRES	PTB	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_10_3364_s_143	11313462	(C) EMSA of c- myc IRES RNA does not show any binding to unr or PTB. (D) EMSA of G3PDH mRNA used a control does not show any binding to unr or PTB.	bind
12196	3	4627	5	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_10_3364_s_143	11313462	(C) EMSA of c- myc IRES RNA does not show any binding to unr or PTB. (D) EMSA of G3PDH mRNA used a control does not show any binding to unr or PTB.	bind
12197	4	4627	5	NULL	NULL	0	NULL	G3PDH mRNA	NULL	control	does not bind	NULL				unr	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_10_3364_s_143	11313462	(C) EMSA of c- myc IRES RNA does not show any binding to unr or PTB. (D) EMSA of G3PDH mRNA used a control does not show any binding to unr or PTB.	bind
12198	5	4627	5	NULL	NULL	0	NULL	G3PDH mRNA	NULL	control	does not bind	NULL				PTB	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_10_3364_s_143	11313462	(C) EMSA of c- myc IRES RNA does not show any binding to unr or PTB. (D) EMSA of G3PDH mRNA used a control does not show any binding to unr or PTB.	bind
12199	6	4627	5	NULL	NULL	0	NULL	statement 4	NULL		is an alternative to	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_10_3364_s_143	11313462	(C) EMSA of c- myc IRES RNA does not show any binding to unr or PTB. (D) EMSA of G3PDH mRNA used a control does not show any binding to unr or PTB.	bind
11711	1	4627	6	NULL	NULL	NULL	NULL	c- myc RNA	NucleicAcid		does not bind				IRES 	unr	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_10_3364_s_143	11313462	(C) EMSA of c- myc IRES RNA does not show any binding to unr or PTB. (D) EMSA of G3PDH mRNA used a control does not show any binding to unr or PTB.	bind
11712	2	4627	6	NULL	NULL	NULL	NULL	c- myc RNA	NucleicAcid		does not bind				IRES	PTB	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_10_3364_s_143	11313462	(C) EMSA of c- myc IRES RNA does not show any binding to unr or PTB. (D) EMSA of G3PDH mRNA used a control does not show any binding to unr or PTB.	bind
11713	3	4627	6	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_10_3364_s_143	11313462	(C) EMSA of c- myc IRES RNA does not show any binding to unr or PTB. (D) EMSA of G3PDH mRNA used a control does not show any binding to unr or PTB.	bind
11714	4	4627	6	NULL	NULL	NULL	NULL	G3PDH mRNA	NucleicAcid		does not bind					unr	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_10_3364_s_143	11313462	(C) EMSA of c- myc IRES RNA does not show any binding to unr or PTB. (D) EMSA of G3PDH mRNA used a control does not show any binding to unr or PTB.	bind
11715	5	4627	6	NULL	NULL	NULL	NULL	G3PDH mRNA	NucleicAcid		does not bind					PTB	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_10_3364_s_143	11313462	(C) EMSA of c- myc IRES RNA does not show any binding to unr or PTB. (D) EMSA of G3PDH mRNA used a control does not show any binding to unr or PTB.	bind
11716	6	4627	6	NULL	NULL	NULL	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_10_3364_s_143	11313462	(C) EMSA of c- myc IRES RNA does not show any binding to unr or PTB. (D) EMSA of G3PDH mRNA used a control does not show any binding to unr or PTB.	bind
12200	1	4628	5	10	NULL	0	NULL	GST-Desrt-ARID	NULL	recombinant	bind	NULL				(TTA)9 oligonucleotide	NULL				NULL		NULL	NULL	NULL	NULL	gw60_genomeres_11_8_1327_s_42	11483573	(C) EMSA of recombinant GST-Desrt-ARID fusion protein binding to a (TTA)9 oligonucleotide (lane  2).	bind
44565	2	4628	5	10	NULL	0	NULL	GST-Desrt-ARID	NULL		is a type of	NULL				fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_genomeres_11_8_1327_s_42	11483573	(C) EMSA of recombinant GST-Desrt-ARID fusion protein binding to a (TTA)9 oligonucleotide (lane  2).	bind
11717	1	4628	6	NULL	NULL	NULL	NULL	GST-Desrt-ARID 	GP	recombinant	bind					(TTA)9 oligonucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genomeres_11_8_1327_s_42	11483573	(C) EMSA of recombinant GST-Desrt-ARID fusion protein binding to a (TTA)9 oligonucleotide (lane  2).	bind
54452	2	4628	6	NULL	NULL	NULL	NULL	GST-Desrt-ARID	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_genomeres_11_8_1327_s_42	11483573	(C) EMSA of recombinant GST-Desrt-ARID fusion protein binding to a (TTA)9 oligonucleotide (lane  2).	bind
12201	1	4629	5	NULL	NULL	0	NULL	ETS-1	NULL	in vitro-translated	bind	NULL				IL-3	NULL			ETS binding site in promoter	NULL		0	NULL	NULL	NULL	gw60_immunity_17_4_437_s_192	12387738	(C) EMSAs demonstrating that in vitro-translated ETS-1 binds to an ETS binding site in the IL-3 promoter (lane 1) but not to the EBS1 (lanes 4-6) or EBS2 (lanes 8-10) sites in the murine perforin promoter.	bind
12202	2	4629	5	NULL	NULL	0	NULL	ETS-1	NULL	in vitro-translated	does not bind	NULL				perforin	NULL	murine		EBS1 sites in promoter	NULL		0	NULL	NULL	NULL	gw60_immunity_17_4_437_s_192	12387738	(C) EMSAs demonstrating that in vitro-translated ETS-1 binds to an ETS binding site in the IL-3 promoter (lane 1) but not to the EBS1 (lanes 4-6) or EBS2 (lanes 8-10) sites in the murine perforin promoter.	bind
12203	3	4629	5	NULL	NULL	0	NULL	ETS-1	NULL	in vitro-translated	does not bind	NULL				perforin	NULL	murine		EBS2 sites in promoter	NULL		0	NULL	NULL	NULL	gw60_immunity_17_4_437_s_192	12387738	(C) EMSAs demonstrating that in vitro-translated ETS-1 binds to an ETS binding site in the IL-3 promoter (lane 1) but not to the EBS1 (lanes 4-6) or EBS2 (lanes 8-10) sites in the murine perforin promoter.	bind
11718	1	4629	6	NULL	NULL	NULL	NULL	ETS-1	GP	in vitro-translated	bind					IL-3	GP			ETS binding site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_4_437_s_192	12387738	(C) EMSAs demonstrating that in vitro-translated ETS-1 binds to an ETS binding site in the IL-3 promoter (lane 1) but not to the EBS1 (lanes 4-6) or EBS2 (lanes 8-10) sites in the murine perforin promoter.	bind
11719	2	4629	6	NULL	NULL	NULL	NULL	ETS-1	GP	in vitro-translated	does not bind					perforin	GP	murine		EBS1 site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_4_437_s_192	12387738	(C) EMSAs demonstrating that in vitro-translated ETS-1 binds to an ETS binding site in the IL-3 promoter (lane 1) but not to the EBS1 (lanes 4-6) or EBS2 (lanes 8-10) sites in the murine perforin promoter.	bind
11720	3	4629	6	NULL	NULL	NULL	NULL	ETS-1	GP	in vitro-translated	does not bind					perforin	GP	murine		EBS2 site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_4_437_s_192	12387738	(C) EMSAs demonstrating that in vitro-translated ETS-1 binds to an ETS binding site in the IL-3 promoter (lane 1) but not to the EBS1 (lanes 4-6) or EBS2 (lanes 8-10) sites in the murine perforin promoter.	bind
12204	1	4630	5	NULL	NULL	0	NULL	CREB	NULL	endogenous	bind	NULL				cpg15	NULL			promoter	NULL	in vivo	0	NULL	NULL	NULL	gw70_molcellneurosci_24_3_538_s_162	14664806	(C) Endogenous CREB binds to the  cpg15 promoter in vivo.	bind
11722	1	4630	6	NULL	NULL	NULL	NULL	CREB	GP	endogenous	bind					cpg15	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellneurosci_24_3_538_s_162	14664806	(C) Endogenous CREB binds to the  cpg15 promoter in vivo.	bind
12205	1	4631	5	NULL	NULL	0	NULL	NGF	NULL	endogenous	bind	NULL	tightly			surface NGF receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_85_3_345_s_93	8616890	(C) Endogenous NGF  is tightly bound to surface NGF receptors.	bind
11723	1	4631	6	NULL	NULL	NULL	NULL	NGF	GP	endogenous	bind		tightly			surface NGF receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_85_3_345_s_93	8616890	(C) Endogenous NGF  is tightly bound to surface NGF receptors.	bind
12207	1	4634	5	NULL	NULL	0	NULL	GDP	NULL		bind	NULL	exclusively			gamma-tubulin	NULL				NULL	in gammaTuSC	NULL	NULL	NULL	NULL	gw60_cellbiol_144_4_721_s_379	10037793	(C) Exclusively, GDP binds to gamma-tubulin in  gammaTuSC (for quantitation see Table  II:  20 muM GDP, experiment 3).	bind
11724	1	4634	6	NULL	NULL	NULL	NULL	GDP	Chemical		bind		exclusively			gamma-tubulin	CellComponent				NULL	gammaTuSC 	NULL	NULL	NULL	NULL	gw60_cellbiol_144_4_721_s_379	10037793	(C) Exclusively, GDP binds to gamma-tubulin in  gammaTuSC (for quantitation see Table  II:  20 muM GDP, experiment 3).	bind
12209	1	4636	5	NULL	NULL	0	NULL	MEKK2	NULL		bind	NULL				Lad	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_7_2298_s_228	12640115	(C) Expression of MEKK2aa228-282 in HEK293 cells blocked MEKK2 binding to Lad. HEK293 cells stably transfected with MEKK2aa228-282, MEKK3aa239-293, or an empty vector were transiently transfected with or without Flag-Lad.	bind
12210	2	4636	5	NULL	NULL	0	NULL	MEKK2	NULL	expression of	blocks	NULL		aa228-282		statement 1	NULL				NULL	in HEK293 cells	0	NULL	NULL	NULL	gw60_molcellbiol_23_7_2298_s_228	12640115	(C) Expression of MEKK2aa228-282 in HEK293 cells blocked MEKK2 binding to Lad. HEK293 cells stably transfected with MEKK2aa228-282, MEKK3aa239-293, or an empty vector were transiently transfected with or without Flag-Lad.	bind
11730	1	4636	6	NULL	NULL	NULL	NULL	MEKK2	GP		bind					Lad	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_7_2298_s_228	12640115	(C) Expression of MEKK2aa228-282 in HEK293 cells blocked MEKK2 binding to Lad. HEK293 cells stably transfected with MEKK2aa228-282, MEKK3aa239-293, or an empty vector were transiently transfected with or without Flag-Lad.	bind
11731	2	4636	6	NULL	NULL	NULL	NULL	MEKK2	GP		expressed in			aa228-282		HEK293 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_7_2298_s_228	12640115	(C) Expression of MEKK2aa228-282 in HEK293 cells blocked MEKK2 binding to Lad. HEK293 cells stably transfected with MEKK2aa228-282, MEKK3aa239-293, or an empty vector were transiently transfected with or without Flag-Lad.	bind
11732	3	4636	6	NULL	NULL	NULL	NULL	statement 2	Process		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_7_2298_s_228	12640115	(C) Expression of MEKK2aa228-282 in HEK293 cells blocked MEKK2 binding to Lad. HEK293 cells stably transfected with MEKK2aa228-282, MEKK3aa239-293, or an empty vector were transiently transfected with or without Flag-Lad.	bind
12211	1	4638	5	NULL	NULL	0	NULL	GI 262570	NULL		bind	NULL				hPPAR	NULL		LBD		NULL		0	NULL	NULL	NULL	gw60_molcell_8_4_737_s_86	11684010	(C) F-L-Leu competes with the binding of GI 262570 to the hPPAR  LBD.	bind
12212	2	4638	5	NULL	NULL	0	NULL		NULL		bind	NULL		F-L-Leu		hPPAR	NULL		LBD		NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_4_737_s_86	11684010	(C) F-L-Leu competes with the binding of GI 262570 to the hPPAR  LBD.	bind
12213	3	4638	5	NULL	NULL	0	NULL	statement 1	NULL		compete with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_8_4_737_s_86	11684010	(C) F-L-Leu competes with the binding of GI 262570 to the hPPAR  LBD.	bind
11733	1	4638	6	NULL	NULL	NULL	NULL	GI 262570	GP		bind					hPPAR	GP		LBD		NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_4_737_s_86	11684010	(C) F-L-Leu competes with the binding of GI 262570 to the hPPAR  LBD.	bind
11734	2	4638	6	NULL	NULL	NULL	NULL				bind			F-L-Leu		hPPAR	GP		LBD		NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_4_737_s_86	11684010	(C) F-L-Leu competes with the binding of GI 262570 to the hPPAR  LBD.	bind
11735	3	4638	6	NULL	NULL	NULL	NULL	statement 1	Process		competes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_4_737_s_86	11684010	(C) F-L-Leu competes with the binding of GI 262570 to the hPPAR  LBD.	bind
12214	1	4639	5	NULL	NULL	0	NULL	curcumin	NULL		bind	NULL				HUVECs	NULL				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_10_8_695_s_120	12954328	(C) FACS analysis of the competitive binding of curcumin with APN-specific antibody (WM15) to HUVECs.	bind
12215	2	4639	5	10	NULL	0	NULL	WM15			is a type of					APN-specific antibody					NULL		NULL	NULL	NULL	NULL	gw60_chembiol_10_8_695_s_120	12954328	(C) FACS analysis of the competitive binding of curcumin with APN-specific antibody (WM15) to HUVECs.	bind
14575	3	4639	5	NULL	NULL	0	NULL	WM15	NULL		bind	NULL				HUVECs	NULL				NULL		0	NULL	NULL	NULL	gw60_chembiol_10_8_695_s_120	12954328	(C) FACS analysis of the competitive binding of curcumin with APN-specific antibody (WM15) to HUVECs.	bind
14576	4	4639	5	NULL	NULL	0	NULL	statement 1	NULL		compete with	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_chembiol_10_8_695_s_120	12954328	(C) FACS analysis of the competitive binding of curcumin with APN-specific antibody (WM15) to HUVECs.	bind
11736	1	4639	6	NULL	NULL	NULL	NULL	curcumin	GP		bind					HUVEC	Cell				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_10_8_695_s_120	12954328	(C) FACS analysis of the competitive binding of curcumin with APN-specific antibody (WM15) to HUVECs.	bind
11737	2	4639	6	NULL	NULL	NULL	NULL	WM15	AminoAcid		bind					HUVEC	Cell				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_10_8_695_s_120	12954328	(C) FACS analysis of the competitive binding of curcumin with APN-specific antibody (WM15) to HUVECs.	bind
11738	3	4639	6	NULL	NULL	NULL	NULL	statement 1	Process		competes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_10_8_695_s_120	12954328	(C) FACS analysis of the competitive binding of curcumin with APN-specific antibody (WM15) to HUVECs.	bind
54461	4	4639	6	NULL	NULL	NULL	NULL	WM15	AminoAcid		is a type of					APN-specific antibody	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_10_8_695_s_120	12954328	(C) FACS analysis of the competitive binding of curcumin with APN-specific antibody (WM15) to HUVECs.	bind
12216	1	4641	5	NULL	NULL	0	NULL	FH	NULL		bind	NULL				Fba	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_11_6206_s_210	12379699	(C) FH binding to Fba is shown.	bind
11739	1	4641	6	NULL	NULL	NULL	NULL	FH	GP		bind					Fba	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_11_6206_s_210	12379699	(C) FH binding to Fba is shown.	bind
12217	1	4642	5	10	NULL	0	NULL	Mia1p-GST		 Filter-immobilized;;recombinant	bind					microtubules		taxol-stabilized			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_5_2212_s_73	16481403	(C) Filter-immobilized  recombinant Mia1p-GST bound taxol-stabilized microtubules in the Far Western assay.	bind
11740	1	4642	6	NULL	NULL	NULL	NULL	Mia1p-GST	GP	Filter-immobilized ;;recombinant	bind					microtubules	CellComponent	taxol-stabilized			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_5_2212_s_73	16481403	(C) Filter-immobilized  recombinant Mia1p-GST bound taxol-stabilized microtubules in the Far Western assay.	bind
12218	1	4644	5	NULL	NULL	0	NULL	FMRP	NULL		bind	NULL				MAP1B mRNA	NULL			5 UTR	NULL		0	NULL	NULL	NULL	gw60_neuron_37_4_555_s_39	12597853	(C) FMRP binds to the 5 UTR of MAP1B mRNA via its G-quartet structure.	bind
12219	2	4644	5	NULL	NULL	0	NULL	statement 1	NULL		via	NULL				G-quartet structure	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_37_4_555_s_39	12597853	(C) FMRP binds to the 5 UTR of MAP1B mRNA via its G-quartet structure.	bind
11741	1	4644	6	NULL	NULL	NULL	NULL	FMRP	GP		bind					MAP1B mRNA	NucleicAcid			5 UTR	NULL		NULL	NULL	NULL	NULL	gw60_neuron_37_4_555_s_39	12597853	(C) FMRP binds to the 5 UTR of MAP1B mRNA via its G-quartet structure.	bind
54462	2	4644	6	NULL	NULL	NULL	NULL	statement 1	Process		via					G-quartet structure					NULL		NULL	NULL	NULL	NULL	gw60_neuron_37_4_555_s_39	12597853	(C) FMRP binds to the 5 UTR of MAP1B mRNA via its G-quartet structure.	bind
12222	1	4647	5	10	NULL	0	NULL	FRS2alpha	NULL		bind	NULL		PTB domain		TrkA	NULL	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_3_979_s_242	10629055	(C) FRS2alpha binds to tyrosine-phosphorylated TrkA via the PTB domain.	bind
11742	1	4647	6	NULL	NULL	NULL	NULL	FRS2alpha	GP		bind			PTB domain		TrkA	GP	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_3_979_s_242	10629055	(C) FRS2alpha binds to tyrosine-phosphorylated TrkA via the PTB domain.	bind
12223	1	4648	5	NULL	NULL	0	NULL	Myc-epsin1	NULL	full-length	is expressed in	NULL				COS cells	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_160_2_213_s_106	12538641	(C) Full-length  Myc-epsin1 and Myc-epsinR expressed in COS cells bind to the GST-appendage domains  of alpha-, beta-, and gamma-adaptin, but not the L762E gamma-adaptin appendage.	bind
12224	2	4648	5	NULL	NULL	0	NULL	Myc-epsinR	NULL	full-length	is expressed in	NULL				COS cells	NULL				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_160_2_213_s_106	12538641	(C) Full-length  Myc-epsin1 and Myc-epsinR expressed in COS cells bind to the GST-appendage domains  of alpha-, beta-, and gamma-adaptin, but not the L762E gamma-adaptin appendage.	bind
12225	3	4648	5	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL				alpha-adaptin	NULL		GST-appendage domains		NULL		0	NULL	NULL	NULL	gw70_cellbiol_160_2_213_s_106	12538641	(C) Full-length  Myc-epsin1 and Myc-epsinR expressed in COS cells bind to the GST-appendage domains  of alpha-, beta-, and gamma-adaptin, but not the L762E gamma-adaptin appendage.	bind
12226	4	4648	5	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL				beta-adaptin	NULL		GST-appendage domains		NULL		0	NULL	NULL	NULL	gw70_cellbiol_160_2_213_s_106	12538641	(C) Full-length  Myc-epsin1 and Myc-epsinR expressed in COS cells bind to the GST-appendage domains  of alpha-, beta-, and gamma-adaptin, but not the L762E gamma-adaptin appendage.	bind
12227	5	4648	5	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL				gamma-adaptin	NULL		GST-appendage domains		NULL		0	NULL	NULL	NULL	gw70_cellbiol_160_2_213_s_106	12538641	(C) Full-length  Myc-epsin1 and Myc-epsinR expressed in COS cells bind to the GST-appendage domains  of alpha-, beta-, and gamma-adaptin, but not the L762E gamma-adaptin appendage.	bind
12228	6	4648	5	NULL	NULL	0	NULL	statement 1	NULL		does not bind	NULL				gamma-adaptin	NULL		L762E appendage		NULL		0	NULL	NULL	NULL	gw70_cellbiol_160_2_213_s_106	12538641	(C) Full-length  Myc-epsin1 and Myc-epsinR expressed in COS cells bind to the GST-appendage domains  of alpha-, beta-, and gamma-adaptin, but not the L762E gamma-adaptin appendage.	bind
12229	7	4648	5	NULL	NULL	0	NULL	statement 2	NULL		bind	NULL				alpha-adaptin	NULL		GST-appendage domains		NULL		0	NULL	NULL	NULL	gw70_cellbiol_160_2_213_s_106	12538641	(C) Full-length  Myc-epsin1 and Myc-epsinR expressed in COS cells bind to the GST-appendage domains  of alpha-, beta-, and gamma-adaptin, but not the L762E gamma-adaptin appendage.	bind
12230	8	4648	5	NULL	NULL	0	NULL	statement 2	NULL		bind	NULL				beta-adaptin	NULL		GST-appendage domains		NULL		0	NULL	NULL	NULL	gw70_cellbiol_160_2_213_s_106	12538641	(C) Full-length  Myc-epsin1 and Myc-epsinR expressed in COS cells bind to the GST-appendage domains  of alpha-, beta-, and gamma-adaptin, but not the L762E gamma-adaptin appendage.	bind
12231	9	4648	5	NULL	NULL	0	NULL	statement 2	NULL		bind	NULL				gamma-adaptin	NULL		GST-appendage domains		NULL		0	NULL	NULL	NULL	gw70_cellbiol_160_2_213_s_106	12538641	(C) Full-length  Myc-epsin1 and Myc-epsinR expressed in COS cells bind to the GST-appendage domains  of alpha-, beta-, and gamma-adaptin, but not the L762E gamma-adaptin appendage.	bind
12232	10	4648	5	NULL	NULL	0	NULL	statement 2	NULL		does not bind	NULL				gamma-adaptin	NULL		L762E appendage		NULL		0	NULL	NULL	NULL	gw70_cellbiol_160_2_213_s_106	12538641	(C) Full-length  Myc-epsin1 and Myc-epsinR expressed in COS cells bind to the GST-appendage domains  of alpha-, beta-, and gamma-adaptin, but not the L762E gamma-adaptin appendage.	bind
11743	1	4648	6	NULL	NULL	NULL	NULL	Myc-epsin1	GP	full length	expressed in					COS cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_160_2_213_s_106	12538641	(C) Full-length  Myc-epsin1 and Myc-epsinR expressed in COS cells bind to the GST-appendage domains  of alpha-, beta-, and gamma-adaptin, but not the L762E gamma-adaptin appendage.	bind
11744	2	4648	6	NULL	NULL	NULL	NULL	statement 1	Process		bind					alpha-adaptin	GP		GST-appendage domain		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_160_2_213_s_106	12538641	(C) Full-length  Myc-epsin1 and Myc-epsinR expressed in COS cells bind to the GST-appendage domains  of alpha-, beta-, and gamma-adaptin, but not the L762E gamma-adaptin appendage.	bind
11745	3	4648	6	NULL	NULL	NULL	NULL	statement 1	Process		bind					beta-adaptin	GP		GST-appendage domain		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_160_2_213_s_106	12538641	(C) Full-length  Myc-epsin1 and Myc-epsinR expressed in COS cells bind to the GST-appendage domains  of alpha-, beta-, and gamma-adaptin, but not the L762E gamma-adaptin appendage.	bind
11746	4	4648	6	NULL	NULL	NULL	NULL	statement 1	Process		bind					gamma-adaptin	GP		GST-appendage domain		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_160_2_213_s_106	12538641	(C) Full-length  Myc-epsin1 and Myc-epsinR expressed in COS cells bind to the GST-appendage domains  of alpha-, beta-, and gamma-adaptin, but not the L762E gamma-adaptin appendage.	bind
11747	5	4648	6	NULL	NULL	NULL	NULL	statement 1	Process		does not bind					gamma-adaptin	GP		L762E appendage		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_160_2_213_s_106	12538641	(C) Full-length  Myc-epsin1 and Myc-epsinR expressed in COS cells bind to the GST-appendage domains  of alpha-, beta-, and gamma-adaptin, but not the L762E gamma-adaptin appendage.	bind
11748	6	4648	6	NULL	NULL	NULL	NULL	Myc-epsinR	GP		expressed in					COS cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_160_2_213_s_106	12538641	(C) Full-length  Myc-epsin1 and Myc-epsinR expressed in COS cells bind to the GST-appendage domains  of alpha-, beta-, and gamma-adaptin, but not the L762E gamma-adaptin appendage.	bind
11749	7	4648	6	NULL	NULL	NULL	NULL	statement 6	Process		bind					alpha-adaptin	GP		GST-appendage domain		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_160_2_213_s_106	12538641	(C) Full-length  Myc-epsin1 and Myc-epsinR expressed in COS cells bind to the GST-appendage domains  of alpha-, beta-, and gamma-adaptin, but not the L762E gamma-adaptin appendage.	bind
11750	8	4648	6	NULL	NULL	NULL	NULL	statement 6	Process		bind					beta-adaptin	GP		GST-appendage domain		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_160_2_213_s_106	12538641	(C) Full-length  Myc-epsin1 and Myc-epsinR expressed in COS cells bind to the GST-appendage domains  of alpha-, beta-, and gamma-adaptin, but not the L762E gamma-adaptin appendage.	bind
11751	9	4648	6	NULL	NULL	NULL	NULL	statement 6	Process		bind					gamma-adaptin	GP		GST-appendage domain		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_160_2_213_s_106	12538641	(C) Full-length  Myc-epsin1 and Myc-epsinR expressed in COS cells bind to the GST-appendage domains  of alpha-, beta-, and gamma-adaptin, but not the L762E gamma-adaptin appendage.	bind
11752	10	4648	6	NULL	NULL	NULL	NULL	statement 6	Process		does not bind					gamma-adaptin	GP		L762E appendage		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_160_2_213_s_106	12538641	(C) Full-length  Myc-epsin1 and Myc-epsinR expressed in COS cells bind to the GST-appendage domains  of alpha-, beta-, and gamma-adaptin, but not the L762E gamma-adaptin appendage.	bind
12243	1	4650	5	NULL	NULL	0	NULL	ARF1	NULL	activated	bind	NULL				cargo proteins	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_168_2_281_s_115	15657398	(C) GAP does not affect the binding of activated ARF1 to cargo proteins.	bind
12244	2	4650	5	NULL	NULL	0	NULL	GAP	NULL		does not affect	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_168_2_281_s_115	15657398	(C) GAP does not affect the binding of activated ARF1 to cargo proteins.	bind
11787	1	4650	6	NULL	NULL	NULL	NULL	ARF1	GP	activated	bind					cargo proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_2_281_s_115	15657398	(C) GAP does not affect the binding of activated ARF1 to cargo proteins.	bind
11789	2	4650	6	NULL	NULL	NULL	NULL	GAP	GP		does not affect					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_2_281_s_115	15657398	(C) GAP does not affect the binding of activated ARF1 to cargo proteins.	bind
12245	2	4652	5	10	NULL	0	NULL	GFP-Wg	NULL		bind	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_development_132_24_5479_s_279	16291792	(C) GFP-Wg binding to S2 cells transfected  with Frizzled2 (top) or Arrow (bottom), as quantified by fluorescence intensity after immunocytochemistry  using an anti-GFP antibody.	bind
44566	1	4652	5	10	NULL	0	NULL	S2 cells	NULL		transfected with	NULL				Frizzled2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_development_132_24_5479_s_279	16291792	(C) GFP-Wg binding to S2 cells transfected  with Frizzled2 (top) or Arrow (bottom), as quantified by fluorescence intensity after immunocytochemistry  using an anti-GFP antibody.	bind
44567	3	4652	5	10	NULL	0	NULL	S2 cells	NULL		transfected with	NULL				Arrow	NULL				NULL		0	NULL	NULL	NULL	gw70_development_132_24_5479_s_279	16291792	(C) GFP-Wg binding to S2 cells transfected  with Frizzled2 (top) or Arrow (bottom), as quantified by fluorescence intensity after immunocytochemistry  using an anti-GFP antibody.	bind
44568	4	4652	5	10	NULL	0	NULL	GFP-Wg	NULL		bind	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_development_132_24_5479_s_279	16291792	(C) GFP-Wg binding to S2 cells transfected  with Frizzled2 (top) or Arrow (bottom), as quantified by fluorescence intensity after immunocytochemistry  using an anti-GFP antibody.	bind
11792	1	4652	6	NULL	NULL	NULL	NULL	S2 cells	Cell		transfected with					Frizzled2	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_132_24_5479_s_279	16291792	(C) GFP-Wg binding to S2 cells transfected  with Frizzled2 (top) or Arrow (bottom), as quantified by fluorescence intensity after immunocytochemistry  using an anti-GFP antibody.	bind
11793	2	4652	6	NULL	NULL	NULL	NULL	S2 cells	Cell		transfected with					Arrow	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_132_24_5479_s_279	16291792	(C) GFP-Wg binding to S2 cells transfected  with Frizzled2 (top) or Arrow (bottom), as quantified by fluorescence intensity after immunocytochemistry  using an anti-GFP antibody.	bind
11794	3	4652	6	NULL	NULL	NULL	NULL	GFP-Wg	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_132_24_5479_s_279	16291792	(C) GFP-Wg binding to S2 cells transfected  with Frizzled2 (top) or Arrow (bottom), as quantified by fluorescence intensity after immunocytochemistry  using an anti-GFP antibody.	bind
11846	4	4652	6	NULL	NULL	NULL	NULL	GFP-Wg	GP		bind					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_132_24_5479_s_279	16291792	(C) GFP-Wg binding to S2 cells transfected  with Frizzled2 (top) or Arrow (bottom), as quantified by fluorescence intensity after immunocytochemistry  using an anti-GFP antibody.	bind
12246	1	4653	5	NULL	NULL	0	NULL	Bfa1	NULL		bind	NULL				Bub2	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_164_2_219_s_179	14734533	(C) Gic1 can disrupt binding between Bfa1 and Bub2.	bind
12247	2	4653	5	NULL	NULL	0	NULL	Gic1	NULL		disrupt	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_164_2_219_s_179	14734533	(C) Gic1 can disrupt binding between Bfa1 and Bub2.	bind
11847	1	4653	6	NULL	NULL	NULL	NULL	Bfa1	GP		bind					Bub2	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_219_s_179	14734533	(C) Gic1 can disrupt binding between Bfa1 and Bub2.	bind
11848	2	4653	6	NULL	NULL	NULL	NULL	Gic1	GP		disrupts					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_219_s_179	14734533	(C) Gic1 can disrupt binding between Bfa1 and Bub2.	bind
12248	1	4654	5	NULL	NULL	0	NULL	GMEB-1	NULL		bind	NULL	specifically			MURF-1	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_157_1_125_s_178	11927605	(C) GMEB-1 specifically binds to MURF-1 in GST pull-down assays.	bind
11849	1	4654	6	NULL	NULL	NULL	NULL	GMEB-1	GP		bind		specifically			MURF-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_1_125_s_178	11927605	(C) GMEB-1 specifically binds to MURF-1 in GST pull-down assays.	bind
12249	1	4658	5	NULL	NULL	0	NULL	Grb-2	NULL		bind	NULL				PY proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_1_26_s_256	11113178	(C) Grb-2 binding with PY proteins.	bind
11851	1	4658	6	NULL	NULL	NULL	NULL	Grb-2	GP		bind					PY proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_1_26_s_256	11113178	(C) Grb-2 binding with PY proteins.	bind
12250	1	4659	5	10	NULL	0	NULL	NF-1			bind					MMTV naked DNA					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_10_3255_s_114	11971959	(C) Greater binding of NF-1 to MMTV naked DNA than to chromatin.	bind
12251	2	4659	5	NULL	NULL	0	NULL	NF-1	NULL		bind	NULL				chromatin	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_10_3255_s_114	11971959	(C) Greater binding of NF-1 to MMTV naked DNA than to chromatin.	bind
12252	3	4659	5	NULL	NULL	0	NULL	statement 1	NULL		greater than	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_10_3255_s_114	11971959	(C) Greater binding of NF-1 to MMTV naked DNA than to chromatin.	bind
11852	1	4659	6	NULL	NULL	NULL	NULL	NF-1	GP		bind					MMTV naked DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_10_3255_s_114	11971959	(C) Greater binding of NF-1 to MMTV naked DNA than to chromatin.	bind
11853	2	4659	6	NULL	NULL	NULL	NULL	NF-1	GP		bind					chromatin	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_10_3255_s_114	11971959	(C) Greater binding of NF-1 to MMTV naked DNA than to chromatin.	bind
11854	3	4659	6	NULL	NULL	NULL	NULL	statement 1	Process		is greater than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_10_3255_s_114	11971959	(C) Greater binding of NF-1 to MMTV naked DNA than to chromatin.	bind
12253	1	4660	5	NULL	NULL	0	NULL	Nup2p	NULL		bind	NULL				Nup60p	NULL				NULL	in yeast extracts	0	NULL	NULL	NULL	gw60_cellbiol_154_5_937_s_123	11535617	(C) Gsp1p - GTP enhances binding of Nup2p to Nup60p in yeast extracts.	bind
12254	2	4660	5	NULL	NULL	0	NULL	Gsp1p - GTP	NULL		enhances	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_154_5_937_s_123	11535617	(C) Gsp1p - GTP enhances binding of Nup2p to Nup60p in yeast extracts.	bind
11855	1	4660	6	NULL	NULL	NULL	NULL	Nup2p	GP		bind					Nup60p	GP				NULL	yeast extracts	NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_937_s_123	11535617	(C) Gsp1p - GTP enhances binding of Nup2p to Nup60p in yeast extracts.	bind
11856	2	4660	6	NULL	NULL	NULL	NULL	Gsp1p - GTP	Chemical		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_937_s_123	11535617	(C) Gsp1p - GTP enhances binding of Nup2p to Nup60p in yeast extracts.	bind
12256	1	4664	5	NULL	NULL	0	NULL	GlyT2	NULL	EGFP-tagged full-length	bind	NULL				GST-syntenin-1	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellneurosci_26_4_518_s_41	15276154	(C) GST pull-down assay showing that EGFP-tagged full-length  GlyT2 bound to GST-syntenin-1, whereas its C-terminal deletion mutant (EGFP-GlyT2  TQC) did not bind.	bind
12257	2	4664	5	NULL	NULL	0	NULL	EGFP-GlyT2 TQC	NULL		is	NULL				C-terminal deletion mutant of EGFP-tagged GlyT2	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellneurosci_26_4_518_s_41	15276154	(C) GST pull-down assay showing that EGFP-tagged full-length  GlyT2 bound to GST-syntenin-1, whereas its C-terminal deletion mutant (EGFP-GlyT2  TQC) did not bind.	bind
12258	3	4664	5	NULL	NULL	0	NULL	EGFP-GlyT2 TQC	NULL		does not bind	NULL				GST-syntenin-1	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellneurosci_26_4_518_s_41	15276154	(C) GST pull-down assay showing that EGFP-tagged full-length  GlyT2 bound to GST-syntenin-1, whereas its C-terminal deletion mutant (EGFP-GlyT2  TQC) did not bind.	bind
11857	1	4664	6	NULL	NULL	NULL	NULL	GlyT2	GP	EGFP-tagged;; full-length	bind					GST-syntenin-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_26_4_518_s_41	15276154	(C) GST pull-down assay showing that EGFP-tagged full-length  GlyT2 bound to GST-syntenin-1, whereas its C-terminal deletion mutant (EGFP-GlyT2  TQC) did not bind.	bind
11858	2	4664	6	NULL	NULL	NULL	NULL	EGFP-GlyT2 TQC	AminoAcid		does not bind					GST-syntenin-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_26_4_518_s_41	15276154	(C) GST pull-down assay showing that EGFP-tagged full-length  GlyT2 bound to GST-syntenin-1, whereas its C-terminal deletion mutant (EGFP-GlyT2  TQC) did not bind.	bind
11859	3	4664	6	NULL	NULL	NULL	NULL	EGFP-GlyT2 TQC	AminoAcid		is					C-terminal deletion mutant EGFP-tagged GlyT2 					NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_26_4_518_s_41	15276154	(C) GST pull-down assay showing that EGFP-tagged full-length  GlyT2 bound to GST-syntenin-1, whereas its C-terminal deletion mutant (EGFP-GlyT2  TQC) did not bind.	bind
12259	1	4666	5	NULL	NULL	0	NULL	GST-FHA	NULL		bind	NULL				Chk2	NULL	activated			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_12_4419_s_71	12024051	(C) GST-FHA binds to activated Chk2.	bind
11860	1	4666	6	NULL	NULL	NULL	NULL	GST-FHA	GP		bind					Chk2	GP	activated			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4419_s_71	12024051	(C) GST-FHA binds to activated Chk2.	bind
12260	1	4670	5	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				DLP1 protein	NULL	WT			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_9_2894_s_195	11553726	(C) GTP binding of DLP1 WT and mutant proteins was tested with the use of GTP as a substrate.	bind
12261	2	4670	5	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				DLP1 protein	NULL	mutant			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_9_2894_s_195	11553726	(C) GTP binding of DLP1 WT and mutant proteins was tested with the use of GTP as a substrate.	bind
11861	1	4670	6	NULL	NULL	NULL	NULL	GTP	Chemical		bind					DLP1	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_9_2894_s_195	11553726	(C) GTP binding of DLP1 WT and mutant proteins was tested with the use of GTP as a substrate.	bind
11862	2	4670	6	NULL	NULL	NULL	NULL	GTP	Chemical		bind					DLP1	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_9_2894_s_195	11553726	(C) GTP binding of DLP1 WT and mutant proteins was tested with the use of GTP as a substrate.	bind
12345	1	4671	5	NULL	NULL	0	NULL	HDAC1	NULL		bind	NULL				Nkx3.2	NULL				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8704_s_144	14612411	(C) HDAC1 binds to Nkx3.2 in a BMP-dependent  manner in vivo.	bind
12346	2	4671	5	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				BMP	NULL				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8704_s_144	14612411	(C) HDAC1 binds to Nkx3.2 in a BMP-dependent  manner in vivo.	bind
11863	1	4671	6	NULL	NULL	NULL	NULL	HDAC1	GP		bind					Nkx3.2	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8704_s_144	14612411	(C) HDAC1 binds to Nkx3.2 in a BMP-dependent  manner in vivo.	bind
11864	2	4671	6	NULL	NULL	NULL	NULL	statement 1	Process		is dependent on					BMP	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8704_s_144	14612411	(C) HDAC1 binds to Nkx3.2 in a BMP-dependent  manner in vivo.	bind
12347	1	4672	5	NULL	NULL	0	NULL	Hip1R	NULL		does not bind	NULL				clathrin HC	NULL		GST-TD (amino acids 1 - 579)		NULL		0	NULL	NULL	NULL	gw60_cellbiol_154_6_1209_s_74	11564758	(c) Hip1R does not bind to GST-TD of clathrin HC (amino acids 1 - 579) immobilized on glutathione-agarose beads (Coomassie stained gel).	bind
11865	1	4672	6	NULL	NULL	NULL	NULL	Hip1R	GP		does not bind					clathrin HC	GP		GST-TD		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_6_1209_s_74	11564758	(c) Hip1R does not bind to GST-TD of clathrin HC (amino acids 1 - 579) immobilized on glutathione-agarose beads (Coomassie stained gel).	bind
12348	1	4675	5	NULL	NULL	0	NULL	Rta	NULL	intact	bind	NULL				BHLF-1	NULL			enhancer	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_12_4390_s_42	12024049	(C) HMGB1 facilitates binding of intact Rta to its sites on the BHLF-1 enhancer.	bind
12349	2	4675	5	NULL	NULL	0	NULL	HMGB1	NULL		facilitate	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_12_4390_s_42	12024049	(C) HMGB1 facilitates binding of intact Rta to its sites on the BHLF-1 enhancer.	bind
11866	1	4675	6	NULL	NULL	NULL	NULL	Rta	GP	intact	bind					BHLF-1	GP			site on enhancer	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4390_s_42	12024049	(C) HMGB1 facilitates binding of intact Rta to its sites on the BHLF-1 enhancer.	bind
11867	2	4675	6	NULL	NULL	NULL	NULL	HMGB1	GP		facilitate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4390_s_42	12024049	(C) HMGB1 facilitates binding of intact Rta to its sites on the BHLF-1 enhancer.	bind
12350	1	4676	5	10	NULL	0	NULL	HNF6			bind					Glut2				promoter	NULL	wild-type chromatin	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7069_s_42	16055718	(c) HNF6 binding to the Glut2 promoter is  13-fold higher in wild-type than in  HNF6 - / -  chromatin, confirming the specificity of the anti-HNF6 antibody.	bind
12351	2	4676	5	10	NULL	0	NULL	HNF6			bind					Glut2					NULL	HNF6 - / - chromatin	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7069_s_42	16055718	(c) HNF6 binding to the Glut2 promoter is  13-fold higher in wild-type than in  HNF6 - / -  chromatin, confirming the specificity of the anti-HNF6 antibody.	bind
12352	3	4676	5	10	NULL	0	NULL	statement 1			is greater than					statement 2					NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7069_s_42	16055718	(c) HNF6 binding to the Glut2 promoter is  13-fold higher in wild-type than in  HNF6 - / -  chromatin, confirming the specificity of the anti-HNF6 antibody.	bind
12353	4	4676	5	10	NULL	0	NULL	statement 3			confirms					anti-HNF6 antibody		specificity of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7069_s_42	16055718	(c) HNF6 binding to the Glut2 promoter is  13-fold higher in wild-type than in  HNF6 - / -  chromatin, confirming the specificity of the anti-HNF6 antibody.	bind
11868	1	4676	6	NULL	NULL	NULL	NULL	HNF6	GP		bind					Glut2	GP			promoter	NULL	wild type chromatin	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7069_s_42	16055718	(c) HNF6 binding to the Glut2 promoter is  13-fold higher in wild-type than in  HNF6 - / -  chromatin, confirming the specificity of the anti-HNF6 antibody.	bind
11869	2	4676	6	NULL	NULL	NULL	NULL	HNF6	GP		bind					Glut2	GP			promoter	NULL	HNF6-/- chromatin	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7069_s_42	16055718	(c) HNF6 binding to the Glut2 promoter is  13-fold higher in wild-type than in  HNF6 - / -  chromatin, confirming the specificity of the anti-HNF6 antibody.	bind
11870	3	4676	6	NULL	NULL	NULL	NULL	statement 1	Process		is greater than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7069_s_42	16055718	(c) HNF6 binding to the Glut2 promoter is  13-fold higher in wild-type than in  HNF6 - / -  chromatin, confirming the specificity of the anti-HNF6 antibody.	bind
54463	4	4676	6	NULL	NULL	NULL	NULL	statement 3	Process		confirms					anti-HNF6 antibody	GP	specificity of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7069_s_42	16055718	(c) HNF6 binding to the Glut2 promoter is  13-fold higher in wild-type than in  HNF6 - / -  chromatin, confirming the specificity of the anti-HNF6 antibody.	bind
12354	1	4678	5	NULL	NULL	0	NULL	HsMAD2	NULL		bind	NULL				GST - TXBP181	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_93_1_81_s_111	9546394	(C) HsMAD2 binds to GST - TXBP181 but not  GST.	bind
12355	2	4678	5	NULL	NULL	0	NULL	HsMAD2	NULL		does not bind	NULL				GST	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_93_1_81_s_111	9546394	(C) HsMAD2 binds to GST - TXBP181 but not  GST.	bind
11871	1	4678	6	NULL	NULL	NULL	NULL	HsMAD2	GP		bind					GST - TXBP181	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_93_1_81_s_111	9546394	(C) HsMAD2 binds to GST - TXBP181 but not  GST.	bind
12356	1	4679	5	NULL	NULL	0	NULL	TGFalpha	NULL	human	bind	NULL				EGF	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_110_6_763_s_91	12297049	(C) Human TGFalpha, EGF, and heparin binding EGF.	bind
12357	2	4679	5	NULL	NULL	0	NULL	EGF	NULL	human	bind	NULL				EGF	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_110_6_763_s_91	12297049	(C) Human TGFalpha, EGF, and heparin binding EGF.	bind
12358	3	4679	5	NULL	NULL	0	NULL	heparin	NULL	human	bind	NULL				EGF	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_110_6_763_s_91	12297049	(C) Human TGFalpha, EGF, and heparin binding EGF.	bind
11873	1	4679	6	NULL	NULL	NULL	NULL	TGFalpha	GP	human	bind					EGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_110_6_763_s_91	12297049	(C) Human TGFalpha, EGF, and heparin binding EGF.	bind
11874	2	4679	6	NULL	NULL	NULL	NULL	EGF	GP	human	bind					EGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_110_6_763_s_91	12297049	(C) Human TGFalpha, EGF, and heparin binding EGF.	bind
11875	3	4679	6	NULL	NULL	NULL	NULL	heparin	GP	human	bind					EGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_110_6_763_s_91	12297049	(C) Human TGFalpha, EGF, and heparin binding EGF.	bind
12359	1	4680	5	NULL	NULL	0	NULL	HVEM	NULL		bind	NULL				LT	NULL				NULL		0	NULL	NULL	NULL	gw60_immunity_8_1_21_s_101	9462508	(C) HVEM binds LT  and gD-1.	bind
12360	2	4680	5	NULL	NULL	0	NULL	HVEM	NULL		bind	NULL				gD-1	NULL				NULL		0	NULL	NULL	NULL	gw60_immunity_8_1_21_s_101	9462508	(C) HVEM binds LT  and gD-1.	bind
11876	1	4680	6	NULL	NULL	NULL	NULL	HVEM	GP		bind					LT	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_8_1_21_s_101	9462508	(C) HVEM binds LT  and gD-1.	bind
11877	2	4680	6	NULL	NULL	NULL	NULL	HVEM	GP		bind					gD-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_8_1_21_s_101	9462508	(C) HVEM binds LT  and gD-1.	bind
12361	1	4682	5	NULL	NULL	0	NULL	IE2	NULL		bind	NULL	directly			Spi-1	NULL		antiparallel beta3 and beta4 of wing motif		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_6803_s_248	10490619	(c) IE2 directly bound to Spi-1 through a portion (antiparallel beta3 and beta4) of the wing motif (lane 6).	bind
11878	1	4682	6	NULL	NULL	NULL	NULL	IE2	GP		bind		directly			Spi-1	GP		antiparallel beta3 and beta4 of the wing motif		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_6803_s_248	10490619	(c) IE2 directly bound to Spi-1 through a portion (antiparallel beta3 and beta4) of the wing motif (lane 6).	bind
12365	1	4684	5	NULL	NULL	0	NULL	FKBP12	NULL		bind	NULL				RyR1	NULL	WT			NULL		0	NULL	NULL	NULL	gw70_cellbiol_160_6_919_s_51	12629052	(C) Immunoblot showing binding of  FKBP12 to WT and mutant RyR1, assessed by centrifugation (FKBP12 cosediments with  RyR1) and FKBP12 immunoblotting.	bind
12366	2	4684	5	NULL	NULL	0	NULL	FKBP12	NULL		bind	NULL				RyR1	NULL	mutant			NULL		0	NULL	NULL	NULL	gw70_cellbiol_160_6_919_s_51	12629052	(C) Immunoblot showing binding of  FKBP12 to WT and mutant RyR1, assessed by centrifugation (FKBP12 cosediments with  RyR1) and FKBP12 immunoblotting.	bind
11879	1	4684	6	NULL	NULL	NULL	NULL	FKBP12	GP		bind					RyR1	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_160_6_919_s_51	12629052	(C) Immunoblot showing binding of  FKBP12 to WT and mutant RyR1, assessed by centrifugation (FKBP12 cosediments with  RyR1) and FKBP12 immunoblotting.	bind
11880	2	4684	6	NULL	NULL	NULL	NULL	FKBP12	GP		bind					RyR1	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_160_6_919_s_51	12629052	(C) Immunoblot showing binding of  FKBP12 to WT and mutant RyR1, assessed by centrifugation (FKBP12 cosediments with  RyR1) and FKBP12 immunoblotting.	bind
12370	1	4685	5	NULL	NULL	0	NULL	anti-PMT polyclonal antibodies	NULL		bind	NULL				peptides	NULL	recombinant			NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_12_7839_s_187	11705966	(C) Immunoblot showing the binding of anti-PMT and anti-peptide polyclonal antibodies to recombinant peptides.	bind
12372	2	4685	5	NULL	NULL	0	NULL	anti-peptide polyclonal antibodies	NULL		bind	NULL				peptides	NULL	recombinant			NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_12_7839_s_187	11705966	(C) Immunoblot showing the binding of anti-PMT and anti-peptide polyclonal antibodies to recombinant peptides.	bind
12375	1	4686	5	NULL	NULL	0	NULL	cyclin E	NULL		bind	NULL				p21	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3916_s_334	10207115	(C) Immunodepletion of cyclin E bound to p21 following 3 days of p16 induction.	bind
12376	2	4686	5	NULL	NULL	0	NULL	p16	NULL	induction	immunodeplete	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3916_s_334	10207115	(C) Immunodepletion of cyclin E bound to p21 following 3 days of p16 induction.	bind
11881	1	4686	6	NULL	NULL	NULL	NULL	cyclin E	GP		bind					p21	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3916_s_334	10207115	(C) Immunodepletion of cyclin E bound to p21 following 3 days of p16 induction.	bind
54464	1	4686	6	NULL	NULL	NULL	NULL	p16	GP	induction of	immunodeplete					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3916_s_334	10207115	(C) Immunodepletion of cyclin E bound to p21 following 3 days of p16 induction.	bind
13428	1	4687	5	NULL	NULL	0	NULL	Rep-kappaBBP-Jkappa	NULL		bind	NULL				NF-kappaB2-specific oligonucleotide	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2077_s_319	9528780	(C) In cell lysates transfected with a Notch-1-IC expression plasmid, Rep-kappaBBP-Jkappa-specific DNA binding activity bound to the NF-kappaB2-specific oligonucleotide (complex A) was abolished, but no higher-order complex, could be identified; it was probably masked by additional NF-kappaB-specific DNA binding activity (complex B).	bind
13431	2	4687	5	10	NULL	0	NULL	Notch-1-IC 	NULL		inhibit	NULL				statement 1	NULL				NULL	cell lysates	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2077_s_319	9528780	(C) In cell lysates transfected with a Notch-1-IC expression plasmid, Rep-kappaBBP-Jkappa-specific DNA binding activity bound to the NF-kappaB2-specific oligonucleotide (complex A) was abolished, but no higher-order complex, could be identified; it was probably masked by additional NF-kappaB-specific DNA binding activity (complex B).	bind
12273	1	4687	6	NULL	NULL	NULL	NULL	Rep-kappaBBP-Jkappa-	GP		bind					NF-kappaB2-specific oligonucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2077_s_319	9528780	(C) In cell lysates transfected with a Notch-1-IC expression plasmid, Rep-kappaBBP-Jkappa-specific DNA binding activity bound to the NF-kappaB2-specific oligonucleotide (complex A) was abolished, but no higher-order complex, could be identified; it was probably masked by additional NF-kappaB-specific DNA binding activity (complex B).	bind
12448	2	4687	6	NULL	NULL	NULL	NULL	Notch-1-IC 	GP		inhibits					statement 1	Process				NULL	cell lysates	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2077_s_319	9528780	(C) In cell lysates transfected with a Notch-1-IC expression plasmid, Rep-kappaBBP-Jkappa-specific DNA binding activity bound to the NF-kappaB2-specific oligonucleotide (complex A) was abolished, but no higher-order complex, could be identified; it was probably masked by additional NF-kappaB-specific DNA binding activity (complex B).	bind
13422	1	4688	5	NULL	NULL	0	NULL		NULL		replaces	NULL			G residue		NULL			A in the lexA binding site upstream of recA	NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_22_6235_s_41	12399494	(C) In the  recA281(Oc) mutation, a G residue replaces A in the  lexA binding site upstream of  recA.	bind
13423	2	4688	5	NULL	NULL	0	NULL	statement 1	NULL		occurs in	NULL				recA281(Oc)	NULL	mutation			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_22_6235_s_41	12399494	(C) In the  recA281(Oc) mutation, a G residue replaces A in the  lexA binding site upstream of  recA.	bind
13406	1	4689	5	10	NULL	0	NULL	GSK-3		inactive	in the presence of					Li+					NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_24_3_673_s_234	14664817	(C) In the presence of Li+ and excess (transfected) Axin, GSK-3 is inactive and protein X is unphosphorylated,  but Axin binds to protein X preventing induction of neurite outgrowth.	bind
13407	2	4689	5	10	NULL	0	NULL	protein X		unphosphorylated	in the presence of					Li+					NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_24_3_673_s_234	14664817	(C) In the presence of Li+ and excess (transfected) Axin, GSK-3 is inactive and protein X is unphosphorylated,  but Axin binds to protein X preventing induction of neurite outgrowth.	bind
13408	3	4689	5	10	NULL	0	NULL	GSK-3		inactive	in the presence of					Axin		excess			NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_24_3_673_s_234	14664817	(C) In the presence of Li+ and excess (transfected) Axin, GSK-3 is inactive and protein X is unphosphorylated,  but Axin binds to protein X preventing induction of neurite outgrowth.	bind
13415	4	4689	5	10	NULL	0	NULL	protein X		unphosphorylated	in the presence of					Axin		excess			NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_24_3_673_s_234	14664817	(C) In the presence of Li+ and excess (transfected) Axin, GSK-3 is inactive and protein X is unphosphorylated,  but Axin binds to protein X preventing induction of neurite outgrowth.	bind
13417	5	4689	5	NULL	NULL	0	NULL	Axin	NULL		bind	NULL				protein X	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellneurosci_24_3_673_s_234	14664817	(C) In the presence of Li+ and excess (transfected) Axin, GSK-3 is inactive and protein X is unphosphorylated,  but Axin binds to protein X preventing induction of neurite outgrowth.	bind
13418	6	4689	5	NULL	NULL	0	NULL	statement 5	NULL		prevents	NULL				neurite outgrowth	NULL	induction of			NULL		0	NULL	NULL	NULL	gw70_molcellneurosci_24_3_673_s_234	14664817	(C) In the presence of Li+ and excess (transfected) Axin, GSK-3 is inactive and protein X is unphosphorylated,  but Axin binds to protein X preventing induction of neurite outgrowth.	bind
11882	1	4689	6	NULL	NULL	NULL	NULL	Axin	GP		bind					protein X	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_24_3_673_s_234	14664817	(C) In the presence of Li+ and excess (transfected) Axin, GSK-3 is inactive and protein X is unphosphorylated,  but Axin binds to protein X preventing induction of neurite outgrowth.	bind
11883	2	4689	6	NULL	NULL	NULL	NULL	statement 1	Process		prevents					neurite outgrowth	Process	induction of 			NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_24_3_673_s_234	14664817	(C) In the presence of Li+ and excess (transfected) Axin, GSK-3 is inactive and protein X is unphosphorylated,  but Axin binds to protein X preventing induction of neurite outgrowth.	bind
12279	3	4689	6	NULL	NULL	NULL	NULL	GSK-3	GP	inactive	in the presence of					Li+	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_24_3_673_s_234	14664817	(C) In the presence of Li+ and excess (transfected) Axin, GSK-3 is inactive and protein X is unphosphorylated,  but Axin binds to protein X preventing induction of neurite outgrowth.	bind
57790	4	4689	6	NULL	NULL	NULL	NULL	protein X	GP	unphosphorylated	in the presence of					Li+	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_24_3_673_s_234	14664817	(C) In the presence of Li+ and excess (transfected) Axin, GSK-3 is inactive and protein X is unphosphorylated,  but Axin binds to protein X preventing induction of neurite outgrowth.	bind
57791	5	4689	6	NULL	NULL	NULL	NULL	GSK-3	GP	inactive	in the presence of					Axin	GP	excess			NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_24_3_673_s_234	14664817	(C) In the presence of Li+ and excess (transfected) Axin, GSK-3 is inactive and protein X is unphosphorylated,  but Axin binds to protein X preventing induction of neurite outgrowth.	bind
57793	6	4689	6	NULL	NULL	NULL	NULL	protein X	GP	unphosphorylated	in the presence of					Axin	GP	excess			NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_24_3_673_s_234	14664817	(C) In the presence of Li+ and excess (transfected) Axin, GSK-3 is inactive and protein X is unphosphorylated,  but Axin binds to protein X preventing induction of neurite outgrowth.	bind
12383	1	4690	5	10	NULL	0	NULL	C-sos1			displace from					 grb2 CH2					NULL	in vitro	NULL	NULL	NULL	NULL	gw70_cellbiol_172_6_817_s_123	16520382	(C) In vitro binding assay showing displacement  of CH2 from grb2 by C-sos1.	bind
11884	1	4690	6	NULL	NULL	NULL	NULL	C-sos1	GP		displace from					grb2 CH2	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_cellbiol_172_6_817_s_123	16520382	(C) In vitro binding assay showing displacement  of CH2 from grb2 by C-sos1.	bind
12384	1	4691	5	NULL	NULL	0	NULL	AP-3	NULL		bind	NULL				AGAP1	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_devcell_5_3_513_s_44	12967569	(C) In vitro binding between AP-3 and GST fusion proteins of AGAP1.	bind
44569	2	4691	5	10	NULL	0	NULL	AGAP1	NULL		is a type of	NULL				GST fusion protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_devcell_5_3_513_s_44	12967569	(C) In vitro binding between AP-3 and GST fusion proteins of AGAP1.	bind
11885	1	4691	6	NULL	NULL	NULL	NULL	AP-3	GP		bind					AGAP1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_devcell_5_3_513_s_44	12967569	(C) In vitro binding between AP-3 and GST fusion proteins of AGAP1.	bind
54467	2	4691	6	NULL	NULL	NULL	NULL	AGAP1	GP		is a type of					GST fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_5_3_513_s_44	12967569	(C) In vitro binding between AP-3 and GST fusion proteins of AGAP1.	bind
12385	1	4692	5	NULL	NULL	0	NULL	S35Metataxin	NULL		bind	NULL		1539-816		p80 coilin	NULL		266-597		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1638_1_35_s_110	12757932	(C) In vitro binding between S35Metataxin-1539-816 and GST-fusion-p80 coilin266-597.	bind
44570	2	4692	5	10	NULL	0	NULL	p80 coilin	NULL		is a type of	NULL		266-597		GST-fusion protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1638_1_35_s_110	12757932	(C) In vitro binding between S35Metataxin-1539-816 and GST-fusion-p80 coilin266-597.	bind
11886	1	4692	6	NULL	NULL	NULL	NULL	S35Metataxin	GP		bind			1539-816		p80 coilin	GP		266-597		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1638_1_35_s_110	12757932	(C) In vitro binding between S35Metataxin-1539-816 and GST-fusion-p80 coilin266-597.	bind
54468	2	4692	6	NULL	NULL	NULL	NULL	p80 coilin	GP		is a type of			266-597		GST fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1638_1_35_s_110	12757932	(C) In vitro binding between S35Metataxin-1539-816 and GST-fusion-p80 coilin266-597.	bind
12387	1	4693	5	NULL	NULL	0	NULL	PaaX	NULL		bind	NULL				Ppac	NULL			promoter	NULL	in vitro	0	NULL	NULL	NULL	gw70_jbacteriol_186_7_2215_s_47	15028709	(C) In vitro binding of PaaX to the  Ppac promoter by gel retardation assay.	bind
11887	1	4693	6	NULL	NULL	NULL	NULL	PaaX	GP		bind					Ppac	GP			promoter	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbacteriol_186_7_2215_s_47	15028709	(C) In vitro binding of PaaX to the  Ppac promoter by gel retardation assay.	bind
12388	1	4694	5	10	NULL	0	NULL	ARF		radiolabeled;;human	bind					GST					NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_4_1258_s_176	15684379	(C) In vitro binding of radiolabeled  human ARF to GST, GST-wild-type NPM (WT), or various GST-NPM mutants (NPM residues  fused to GST are indicated) was detected by autoradiography.	bind
12389	2	4694	5	10	NULL	0	NULL	ARF		radiolabeled;;human	bind					GST- NPM		wild-type			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_4_1258_s_176	15684379	(C) In vitro binding of radiolabeled  human ARF to GST, GST-wild-type NPM (WT), or various GST-NPM mutants (NPM residues  fused to GST are indicated) was detected by autoradiography.	bind
12390	3	4694	5	10	NULL	0	NULL	ARF		radiolabeled;;human	bind					GST-NPM		mutant			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_4_1258_s_176	15684379	(C) In vitro binding of radiolabeled  human ARF to GST, GST-wild-type NPM (WT), or various GST-NPM mutants (NPM residues  fused to GST are indicated) was detected by autoradiography.	bind
11888	1	4694	6	NULL	NULL	NULL	NULL	ARF	GP	radiolabeled;; human	bind					GST					NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_4_1258_s_176	15684379	(C) In vitro binding of radiolabeled  human ARF to GST, GST-wild-type NPM (WT), or various GST-NPM mutants (NPM residues  fused to GST are indicated) was detected by autoradiography.	bind
11889	2	4694	6	NULL	NULL	NULL	NULL	ARF	GP	radiolabeled;; human	bind					GST-NPM	GP	wild type			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_4_1258_s_176	15684379	(C) In vitro binding of radiolabeled  human ARF to GST, GST-wild-type NPM (WT), or various GST-NPM mutants (NPM residues  fused to GST are indicated) was detected by autoradiography.	bind
11890	3	4694	6	NULL	NULL	NULL	NULL	ARF	GP	radiolabeled;; human	bind					GST-NPM	GP	mutant			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_4_1258_s_176	15684379	(C) In vitro binding of radiolabeled  human ARF to GST, GST-wild-type NPM (WT), or various GST-NPM mutants (NPM residues  fused to GST are indicated) was detected by autoradiography.	bind
12392	1	4696	5	NULL	NULL	0	NULL	Src	NULL		bind	NULL				RACK1	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_6_3245_s_206	9584165	(C) In vitro protein kinase activity of Src bound to RACK1.	bind
11891	1	4696	6	NULL	NULL	NULL	NULL	Src	GP		bind					RACK1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_6_3245_s_206	9584165	(C) In vitro protein kinase activity of Src bound to RACK1.	bind
12395	1	4699	5	NULL	NULL	0	NULL	HIRA protein	NULL	in vitro-labeled	bind	NULL				core histone H4	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_9_5546_s_193	9710638	(C) In vitro-labeled HIRA protein binds core histone H4 immobilized on beads.	bind
11892	1	4699	6	NULL	NULL	NULL	NULL	HIRA	GP	In vitro-labeled 	bind					core histone H4	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5546_s_193	9710638	(C) In vitro-labeled HIRA protein binds core histone H4 immobilized on beads.	bind
12396	1	4700	5	NULL	NULL	0	NULL	IRF-1	NULL		bind	NULL				IL-4	NULL			promoter	NULL	in vivo in peripheral blood T cells 	NULL	NULL	NULL	NULL	gw60_immunity_17_6_703_s_189	12479817	(C) In vivo binding of IRF-1 and IRF-2 to the IL-4 promoter in peripheral blood T cells upon IFN-  stimulation.	bind
12397	2	4700	5	NULL	NULL	0	NULL	statement 1	NULL		occurs upon	NULL				IFN	NULL	stimulation			NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_6_703_s_189	12479817	(C) In vivo binding of IRF-1 and IRF-2 to the IL-4 promoter in peripheral blood T cells upon IFN-  stimulation.	bind
12398	3	4700	5	NULL	NULL	0	NULL	IRF-2	NULL		bind	NULL				IL-4	NULL			promoter	NULL	in vivo in peripheral blood T cells	0	NULL	NULL	NULL	gw60_immunity_17_6_703_s_189	12479817	(C) In vivo binding of IRF-1 and IRF-2 to the IL-4 promoter in peripheral blood T cells upon IFN-  stimulation.	bind
12399	4	4700	5	NULL	NULL	0	NULL	statement 3	NULL		occurs upon	NULL				IFN	NULL	stimulation			NULL		0	NULL	NULL	NULL	gw60_immunity_17_6_703_s_189	12479817	(C) In vivo binding of IRF-1 and IRF-2 to the IL-4 promoter in peripheral blood T cells upon IFN-  stimulation.	bind
11893	1	4700	6	NULL	NULL	NULL	NULL	IRF-1	GP		bind					IL-4	GP			promoter	NULL	peripheral blood T cells, in vivo	NULL	NULL	NULL	NULL	gw60_immunity_17_6_703_s_189	12479817	(C) In vivo binding of IRF-1 and IRF-2 to the IL-4 promoter in peripheral blood T cells upon IFN-  stimulation.	bind
11894	2	4700	6	NULL	NULL	NULL	NULL	IRF-2	GP		bind					IL-4	GP			promoter	NULL	peripheral blood T cells, in vivo	NULL	NULL	NULL	NULL	gw60_immunity_17_6_703_s_189	12479817	(C) In vivo binding of IRF-1 and IRF-2 to the IL-4 promoter in peripheral blood T cells upon IFN-  stimulation.	bind
11895	3	4700	6	NULL	NULL	NULL	NULL	IFN	GP		stimulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_6_703_s_189	12479817	(C) In vivo binding of IRF-1 and IRF-2 to the IL-4 promoter in peripheral blood T cells upon IFN-  stimulation.	bind
11896	4	4700	6	NULL	NULL	NULL	NULL	IFN	GP		stimulates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_6_703_s_189	12479817	(C) In vivo binding of IRF-1 and IRF-2 to the IL-4 promoter in peripheral blood T cells upon IFN-  stimulation.	bind
12400	1	4701	5	NULL	NULL	0	NULL	SATB1	NULL		bind	NULL				IL-2	NULL	distal		promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1620_s_182	15713622	(C) In vivo binding of SATB1 to  the distal IL-2 promoter.	bind
11897	1	4701	6	NULL	NULL	NULL	NULL	SATB1	GP		bind					IL-2	GP	distal		promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1620_s_182	15713622	(C) In vivo binding of SATB1 to  the distal IL-2 promoter.	bind
13229	1	4702	5	NULL	NULL	0	NULL	PDX-1	NULL	endogenous	bind	NULL				LRH-1	NULL	murine		promoter	NULL	in the gut from E13.5 embryos	0	NULL	NULL	NULL	gw70_molcellbiol_23_19_6713_s_189	12972592	(C) In vivo ChIP assay demonstrating  binding of endogenous PDX-1 to the murine LRH-1 promoter in the gut and pancreas  from E13.5 embryos.	bind
13230	2	4702	5	NULL	NULL	0	NULL	PDX-1	NULL	endogenous	bind	NULL				LRH-1	NULL	murine		promoter	NULL	in the pancreas from E13.5 embryos	0	NULL	NULL	NULL	gw70_molcellbiol_23_19_6713_s_189	12972592	(C) In vivo ChIP assay demonstrating  binding of endogenous PDX-1 to the murine LRH-1 promoter in the gut and pancreas  from E13.5 embryos.	bind
11898	1	4702	6	NULL	NULL	NULL	NULL	PDX-1	GP	endogenous	bind					LRH-1	GP	murine		promoter	NULL	gut from E13.5 embryos	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_19_6713_s_189	12972592	(C) In vivo ChIP assay demonstrating  binding of endogenous PDX-1 to the murine LRH-1 promoter in the gut and pancreas  from E13.5 embryos.	bind
15183	2	4702	6	NULL	NULL	NULL	NULL	PDX-1	GP	endogenous	bind					LRH-1	GP	murine		promoter	NULL	pancreas from E13.5 embryos	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_19_6713_s_189	12972592	(C) In vivo ChIP assay demonstrating  binding of endogenous PDX-1 to the murine LRH-1 promoter in the gut and pancreas  from E13.5 embryos.	bind
13231	1	4703	5	NULL	NULL	0	NULL	beta3-integrin	NULL		induce	NULL				PEA3	NULL	DNA-binding activity of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_6_2118_s_219	11238946	(C) Induction of PEA3 DNA-binding activity by beta3-integrin.	bind
11900	1	4703	6	NULL	NULL	NULL	NULL	beta3-integrin	GP		induces					PEA3	GP	DNA binding activity of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_6_2118_s_219	11238946	(C) Induction of PEA3 DNA-binding activity by beta3-integrin.	bind
13232	1	4704	5	NULL	NULL	0	NULL	BMP4	NULL		bind	NULL				BMPR1B	NULL		ectodomain		NULL		0	NULL	NULL	NULL	gw70_development_131_1_229_s_146	14660436	(C) Inhibition of BMP4 binding to BMPR1B  ectodomain by mCHL2-FLAG.	bind
13233	2	4704	5	NULL	NULL	0	NULL	mCHL2-FLAG	NULL		inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_development_131_1_229_s_146	14660436	(C) Inhibition of BMP4 binding to BMPR1B  ectodomain by mCHL2-FLAG.	bind
11901	1	4704	6	NULL	NULL	NULL	NULL	BMP4	GP		bind					BMPR1B	GP		ectodomain		NULL		NULL	NULL	NULL	NULL	gw70_development_131_1_229_s_146	14660436	(C) Inhibition of BMP4 binding to BMPR1B  ectodomain by mCHL2-FLAG.	bind
11902	2	4704	6	NULL	NULL	NULL	NULL	mCHL2-FLAG	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_131_1_229_s_146	14660436	(C) Inhibition of BMP4 binding to BMPR1B  ectodomain by mCHL2-FLAG.	bind
13234	1	4705	5	NULL	NULL	0	NULL	Ac-DEVD-CHO	NULL		inhibit	NULL				eIF4G	NULL	cleavage of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_12_7565_s_279	9819442	(C) Inhibition of eIF4G cleavage by Ac-DEVD-CHO.	bind
11903	1	4705	6	NULL	NULL	NULL	NULL	Ac-DEVD-CHO	GP		inhibits					eIF4G	GP	clevage of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7565_s_279	9819442	(C) Inhibition of eIF4G cleavage by Ac-DEVD-CHO.	bind
13235	1	4706	5	NULL	NULL	0	NULL	Gt	NULL		bind	NULL				rhodopsin	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_3_5_649_s_56	10360181	(C) Inhibition of Gt binding to rhodopsin by phosducin.	bind
13236	2	4706	5	NULL	NULL	0	NULL	phosducin	NULL		inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_3_5_649_s_56	10360181	(C) Inhibition of Gt binding to rhodopsin by phosducin.	bind
11904	1	4706	6	NULL	NULL	NULL	NULL	Gt	GP		bind					rhodopsin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_5_649_s_56	10360181	(C) Inhibition of Gt binding to rhodopsin by phosducin.	bind
11905	2	4706	6	NULL	NULL	NULL	NULL	phosducin	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_5_649_s_56	10360181	(C) Inhibition of Gt binding to rhodopsin by phosducin.	bind
13237	1	4707	5	NULL	NULL	0	NULL	anti-BSAP antibody	NULL		inhibit	NULL				NF-JC	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw60_immunity_5_4_377_s_97	8885870	(C) Inhibition of NF-JC binding by anti-BSAP antibody.	bind
11906	1	4707	6	NULL	NULL	NULL	NULL	anti-BSAP antibody	GP		inhibits					NF-JC	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_immunity_5_4_377_s_97	8885870	(C) Inhibition of NF-JC binding by anti-BSAP antibody.	bind
13238	2	4708	5	10	NULL	NULL	NULL	7-Cl-Kyn	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_110_2_159_s_146	12591153	(C) Inhibition of NMDA receptor-mediated currents by 7-Cl-Kyn, a competitive antagonist of NMDA receptors acting on the glycine binding site of NR1.	bind
13239	4	4708	5	10	NULL	NULL	NULL	7-Cl-Kyn	Chemical		is					NMDA receptors	GP	competitive antagonist of 			NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_110_2_159_s_146	12591153	(C) Inhibition of NMDA receptor-mediated currents by 7-Cl-Kyn, a competitive antagonist of NMDA receptors acting on the glycine binding site of NR1.	bind
13240	3	4708	5	10	NULL	NULL	NULL	7-Cl-Kyn	Chemical		acts on					NR1	GP		glycine binding site 		NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_110_2_159_s_146	12591153	(C) Inhibition of NMDA receptor-mediated currents by 7-Cl-Kyn, a competitive antagonist of NMDA receptors acting on the glycine binding site of NR1.	bind
54477	1	4708	5	10	NULL	NULL	NULL	NMDA receptor	GP		mediates					currents	AbstractConcept				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_110_2_159_s_146	12591153	(C) Inhibition of NMDA receptor-mediated currents by 7-Cl-Kyn, a competitive antagonist of NMDA receptors acting on the glycine binding site of NR1.	bind
12278	1	4708	6	10	NULL	NULL	NULL	NMDA receptors	GP		mediates					currents	AbstractConcept				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_110_2_159_s_146	12591153	(C) Inhibition of NMDA receptor-mediated currents by 7-Cl-Kyn, a competitive antagonist of NMDA receptors acting on the glycine binding site of NR1.	bind
12449	2	4708	6	10	NULL	NULL	NULL	7-Cl-Kyn	Chemical		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_110_2_159_s_146	12591153	(C) Inhibition of NMDA receptor-mediated currents by 7-Cl-Kyn, a competitive antagonist of NMDA receptors acting on the glycine binding site of NR1.	bind
12450	3	4708	6	NULL	NULL	NULL	NULL	7-Cl-Kyn	Chemical		is					NMDA receptors	GP	competitive antagonist of 			NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_110_2_159_s_146	12591153	(C) Inhibition of NMDA receptor-mediated currents by 7-Cl-Kyn, a competitive antagonist of NMDA receptors acting on the glycine binding site of NR1.	bind
12451	4	4708	6	NULL	NULL	NULL	NULL	7-Cl-Kyn	Chemical		acts on					NR1	GP		glycine binding site		NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_110_2_159_s_146	12591153	(C) Inhibition of NMDA receptor-mediated currents by 7-Cl-Kyn, a competitive antagonist of NMDA receptors acting on the glycine binding site of NR1.	bind
13241	1	4709	5	NULL	NULL	0	NULL	LLN	NULL		is	NULL				LLNL	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_24_9236_s_230	11094075	(C) Inhibition of proteasome by LLNL (LLN) stabilizes p27Kip1 protein levels.	bind
13242	2	4709	5	NULL	NULL	0	NULL		NULL		inhibit	NULL		LLN		proteasome	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_24_9236_s_230	11094075	(C) Inhibition of proteasome by LLNL (LLN) stabilizes p27Kip1 protein levels.	bind
13243	3	4709	5	NULL	NULL	0	NULL	statement 2	NULL		stabilize	NULL				p27Kip1	NULL	protein levels of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_24_9236_s_230	11094075	(C) Inhibition of proteasome by LLNL (LLN) stabilizes p27Kip1 protein levels.	bind
12280	1	4709	6	NULL	NULL	NULL	NULL				inhibits			LLNL		proteasome	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_24_9236_s_230	11094075	(C) Inhibition of proteasome by LLNL (LLN) stabilizes p27Kip1 protein levels.	bind
12281	2	4709	6	NULL	NULL	NULL	NULL	statement 1	Process		stabilizes					p27Kip1	GP	protein levels of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_24_9236_s_230	11094075	(C) Inhibition of proteasome by LLNL (LLN) stabilizes p27Kip1 protein levels.	bind
54478	3	4709	6	10	NULL	0	NULL	LLN			is					LLNL					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_24_9236_s_230	11094075	(C) Inhibition of proteasome by LLNL (LLN) stabilizes p27Kip1 protein levels.	bind
13403	1	4710	5	NULL	NULL	0	NULL	Ras activation	NULL	inhibition of	does not block	NULL					NULL	induction of		RNA Pol I-dependent promoter	NULL	in cells overexpressing TBP	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7086_s_202	9819395	(C) Inhibition of Ras activation does not block induction of RNA Pol I-dependent promoters in cells overexpressing TBP.	bind
15184	1	4710	6	10	NULL	0	NULL	Ras activation		inhibition of	does not block							induction of 		RNA Pol I-dependent promoter	NULL	cells overexpressing TBP	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7086_s_202	9819395	(C) Inhibition of Ras activation does not block induction of RNA Pol I-dependent promoters in cells overexpressing TBP.	bind
13244	1	4711	5	NULL	NULL	0	NULL	Idax	NULL		bind	NULL				Dvl	NULL				NULL	in intact cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_1_330_s_205	11113207	(C) Inhibition of the binding of Idax to Dvl by Axin in intact cells.	bind
13245	2	4711	5	NULL	NULL	0	NULL	Axin	NULL		inhibit	NULL				statement 1	NULL				NULL	in intact cells	0	NULL	NULL	NULL	gw60_molcellbiol_21_1_330_s_205	11113207	(C) Inhibition of the binding of Idax to Dvl by Axin in intact cells.	bind
11907	1	4711	6	NULL	NULL	NULL	NULL	Idax	GP		bind					Dvl	GP				NULL	intact cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_1_330_s_205	11113207	(C) Inhibition of the binding of Idax to Dvl by Axin in intact cells.	bind
11908	2	4711	6	NULL	NULL	NULL	NULL	Axin	GP		inhibits					statement 1	Process				NULL	intact cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_1_330_s_205	11113207	(C) Inhibition of the binding of Idax to Dvl by Axin in intact cells.	bind
13246	1	4712	5	NULL	NULL	0	NULL	Ubc13/Uev1A	NULL	interference of	inhibit	NULL				NF- B	NULL	activation of			NULL	in cells	0	NULL	NULL	NULL	gw60_cell_103_2_351_s_160	11057907	(C) Interference of Ubc13/Uev1A inhibits NF- B activation in cells.	bind
11909	1	4712	6	NULL	NULL	NULL	NULL	Ubc13/Uev1A	GP	Interference of	inhibits					NF-B	GP	activation of			NULL	in cells	NULL	NULL	NULL	NULL	gw60_cell_103_2_351_s_160	11057907	(C) Interference of Ubc13/Uev1A inhibits NF- B activation in cells.	bind
13247	1	4713	5	NULL	NULL	0	NULL	JAK2	NULL		bind	NULL	directly			EpoR	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_8_6_1327_s_109	11779507	(C) JAK2 and JAK2 (JH3-JH7) bind EpoR directly.	bind
13248	2	4713	5	NULL	NULL	0	NULL	JAK2	NULL		bind	NULL	directly	JH3-JH7		EpoR	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_8_6_1327_s_109	11779507	(C) JAK2 and JAK2 (JH3-JH7) bind EpoR directly.	bind
11910	1	4713	6	NULL	NULL	NULL	NULL	JAK2	GP		bind		directly			EpoR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_6_1327_s_109	11779507	(C) JAK2 and JAK2 (JH3-JH7) bind EpoR directly.	bind
11911	2	4713	6	NULL	NULL	NULL	NULL	JAK2	GP		bind		directly	JH3-JH7		EpoR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_6_1327_s_109	11779507	(C) JAK2 and JAK2 (JH3-JH7) bind EpoR directly.	bind
13249	1	4715	5	NULL	NULL	0	NULL	rhodanese 	NULL	[35]methionine-labeled 	bind	NULL				GroEL	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_90_3_491_s_117	9267029	(C) Kinetics of binding and release of [35]methionine-labeled rhodanese and CAT from GroEL.	bind
13250	2	4715	5	NULL	NULL	0	NULL	rhodanese	NULL	[35]methionine-labeled	release	NULL				GroEL	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_90_3_491_s_117	9267029	(C) Kinetics of binding and release of [35]methionine-labeled rhodanese and CAT from GroEL.	bind
13251	3	4715	5	NULL	NULL	0	NULL	CAT	NULL	[35]methionine-labeled	bind	NULL				GroEL	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_90_3_491_s_117	9267029	(C) Kinetics of binding and release of [35]methionine-labeled rhodanese and CAT from GroEL.	bind
13252	4	4715	5	NULL	NULL	0	NULL	CAT	NULL	[35]methionine-labeled	release	NULL				GroEL	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_90_3_491_s_117	9267029	(C) Kinetics of binding and release of [35]methionine-labeled rhodanese and CAT from GroEL.	bind
16234	1	4715	6	NULL	NULL	NULL	NULL	rhodanese	GP	[35]methionine-labeled	bind					GroEL	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_90_3_491_s_117	9267029	(C) Kinetics of binding and release of [35]methionine-labeled rhodanese and CAT from GroEL.	bind
16235	2	4715	6	NULL	NULL	NULL	NULL	rhodanese	GP	[35]methionine-labeled	release					GroEL	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_90_3_491_s_117	9267029	(C) Kinetics of binding and release of [35]methionine-labeled rhodanese and CAT from GroEL.	bind
16237	3	4715	6	NULL	NULL	NULL	NULL	CAT	GP	[35]methionine-labeled	bind					GroEL	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_90_3_491_s_117	9267029	(C) Kinetics of binding and release of [35]methionine-labeled rhodanese and CAT from GroEL.	bind
54479	4	4715	6	NULL	NULL	NULL	NULL	CAT	GP	[35]methionine-labeled	release					GroEL	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_90_3_491_s_117	9267029	(C) Kinetics of binding and release of [35]methionine-labeled rhodanese and CAT from GroEL.	bind
13253	1	4716	5	NULL	NULL	0	NULL	Krox-20	NULL		inhibit	NULL				Schwann cell	NULL	death of			NULL		0	NULL	NULL	NULL	gw70_cellbiol_164_3_385_s_66	14757751	(C) Krox-20 inhibits Schwann cell death after serum withdrawal.	bind
13254	2	4716	5	NULL	NULL	0	NULL	statement 1	NULL		occurs after	NULL				serum	NULL	withdrawal of			NULL		0	NULL	NULL	NULL	gw70_cellbiol_164_3_385_s_66	14757751	(C) Krox-20 inhibits Schwann cell death after serum withdrawal.	bind
11912	1	4716	6	NULL	NULL	NULL	NULL	Krox-20	GP		inhibits					Schwann cell	Cell	death of			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_3_385_s_66	14757751	(C) Krox-20 inhibits Schwann cell death after serum withdrawal.	bind
15185	2	4716	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs after					serum 	OrganismPart	withdrawal of			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_3_385_s_66	14757751	(C) Krox-20 inhibits Schwann cell death after serum withdrawal.	bind
13255	1	4717	5	NULL	NULL	0	NULL	trypomastigote	NULL	T. cruzi	bind	NULL				CASM cells	NULL	human			NULL		0	NULL	NULL	NULL	gw70_infectimmun_72_11_6717_s_49	15501810	(C) Lactose, but not sucrose, inhibits  T. cruzi trypomastigote binding to human CASM cells.	bind
13256	2	4717	5	NULL	NULL	0	NULL	lactose	NULL		inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_72_11_6717_s_49	15501810	(C) Lactose, but not sucrose, inhibits  T. cruzi trypomastigote binding to human CASM cells.	bind
13257	3	4717	5	NULL	NULL	0	NULL	sucrose	NULL		does not inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_72_11_6717_s_49	15501810	(C) Lactose, but not sucrose, inhibits  T. cruzi trypomastigote binding to human CASM cells.	bind
11913	1	4717	6	NULL	NULL	NULL	NULL	trypomastigote	OrganismPart	T. cruzi	bind					CASM cells	Cell	human			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_11_6717_s_49	15501810	(C) Lactose, but not sucrose, inhibits  T. cruzi trypomastigote binding to human CASM cells.	bind
11914	2	4717	6	NULL	NULL	NULL	NULL	lactose	Chemical		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_11_6717_s_49	15501810	(C) Lactose, but not sucrose, inhibits  T. cruzi trypomastigote binding to human CASM cells.	bind
11915	3	4717	6	NULL	NULL	NULL	NULL	sucrose	Chemical		does not inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_11_6717_s_49	15501810	(C) Lactose, but not sucrose, inhibits  T. cruzi trypomastigote binding to human CASM cells.	bind
13825	1	4718	5	10	NULL	0	NULL	TIF2			bind			coactivator motif		GST-GR			LBD		NULL		NULL	NULL	NULL	NULL	gw60_cell_110_1_93_s_68	12151000	(C) Ligand-dependent binding of TIF2 coactivator motif to GST-GR LBD in the presence of a 5-fold excess of dexamethasone (triangles), RU486 (squares), and no compound (circles) was measured by surface plasmon resonance.	bind
54480	2	4718	5	10	NULL	0	NULL	statement 1			depends on					ligand					NULL		NULL	NULL	NULL	NULL	gw60_cell_110_1_93_s_68	12151000	(C) Ligand-dependent binding of TIF2 coactivator motif to GST-GR LBD in the presence of a 5-fold excess of dexamethasone (triangles), RU486 (squares), and no compound (circles) was measured by surface plasmon resonance.	bind
11916	1	4718	6	NULL	NULL	NULL	NULL	TIF2	GP		bind			coactivator motif		GST-GR	GP		LBD		NULL		NULL	NULL	NULL	NULL	gw60_cell_110_1_93_s_68	12151000	(C) Ligand-dependent binding of TIF2 coactivator motif to GST-GR LBD in the presence of a 5-fold excess of dexamethasone (triangles), RU486 (squares), and no compound (circles) was measured by surface plasmon resonance.	bind
11917	2	4718	6	NULL	NULL	NULL	NULL	statement 1	Process		is dependent on					ligand					NULL		NULL	NULL	NULL	NULL	gw60_cell_110_1_93_s_68	12151000	(C) Ligand-dependent binding of TIF2 coactivator motif to GST-GR LBD in the presence of a 5-fold excess of dexamethasone (triangles), RU486 (squares), and no compound (circles) was measured by surface plasmon resonance.	bind
13830	1	4719	5	NULL	NULL	0	NULL	MAb 24c5	NULL		bind	NULL				MTB	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
13831	2	4719	5	NULL	NULL	0	NULL	MTB	NULL		is	NULL				M. tuberculosis Erdman day-20 7H9 medium 	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
13833	3	4719	5	NULL	NULL	0	NULL	MAb 24c5	NULL		bind	NULL				INTPHSE	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
13834	4	4719	5	10	NULL	0	NULL	INTPHSE			is a type of					cell culture supernatant extract					NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
13837	5	4719	5	NULL	NULL	0	NULL	MAb 24c5	NULL		bind	NULL				GC	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
13838	6	4719	5	NULL	NULL	0	NULL	MAb 24c5	NULL		bind	NULL				AM	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
13839	7	4719	5	NULL	NULL	0	NULL	MAb 24c5	NULL		bind	NULL				LAM	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
13840	8	4719	5	NULL	NULL	0	NULL	LAM	NULL		is	NULL				lipoarabinomannan	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
13841	9	4719	5	NULL	NULL	0	NULL	MAb 24c5	NULL		bind	NULL				PIM	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
13842	10	4719	5	NULL	NULL	0	NULL	PIM	NULL		is	NULL				phosphatidylinositol mannoside	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
13843	11	4719	5	NULL	NULL	0	NULL	MAb 24c5	NULL		bind	NULL				LM	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
13844	12	4719	5	NULL	NULL	0	NULL	LM	NULL		is	NULL				fast-growing mycobacterial lipomannan	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
13845	13	4719	5	NULL	NULL	0	NULL	MAb 24c5	NULL		bind	NULL				mAGP	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
13846	14	4719	5	NULL	NULL	0	NULL	mAGP	NULL		is	NULL				mycolyl-arabinogalactan-peptidoglycan complex	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
13847	15	4719	5	NULL	NULL	0	NULL	MAb 24c5	NULL		bind	NULL				TLF	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
13848	16	4719	5	NULL	NULL	0	NULL	TLF	NULL		is	NULL				total lipid fraction	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
12282	1	4719	6	NULL	NULL	NULL	NULL	MAb 24c5	GP		bind					MTB					NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
12283	2	4719	6	NULL	NULL	0	NULL	MTB	NULL		is	NULL				Erdman day-20 7H9 medium	NULL	M. tuberculosis			NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
12285	3	4719	6	NULL	NULL	NULL	NULL	MAb 24c5	GP		bind					INTPHSE					NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
12286	4	4719	6	10	NULL	0	NULL	INTPHSE			is a type of					cell culture supernatant extract 					NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
12287	5	4719	6	NULL	NULL	NULL	NULL	MAb 24c5	GP		bind					GC	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
12288	6	4719	6	NULL	NULL	NULL	NULL	MAb 24c5	GP		bind					AM	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
12289	7	4719	6	NULL	NULL	NULL	NULL	MAb 24c5	GP		bind					LAM	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
12290	8	4719	6	NULL	NULL	NULL	NULL	LAM	Chemical		is					lipoarabinomannan	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
12291	9	4719	6	NULL	NULL	NULL	NULL	MAb 24c5	GP		bind					PIM	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
12292	10	4719	6	NULL	NULL	NULL	NULL	PIM	Chemical		is					phosphatidylinositol mannoside	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
12293	11	4719	6	NULL	NULL	NULL	NULL	MAb 24c5	GP		bind					LM	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
12294	12	4719	6	NULL	NULL	NULL	NULL	LM	Chemical		is					fast-growing mycobacterial lipomannan	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
12295	13	4719	6	NULL	NULL	NULL	NULL	MAb 24c5	GP		bind					mAGP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
12296	14	4719	6	NULL	NULL	NULL	NULL	mAGP	Chemical		is					mycolyl-arabinogalactan-peptidoglycan complex	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
12297	15	4719	6	NULL	NULL	NULL	NULL	MAb 24c5	GP		bind					TLF	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
12298	16	4719	6	NULL	NULL	NULL	NULL	TLF	OrganismPart		is					total lipid fraction	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_145	11953397	(C) MAb 24c5 binding to  M. tuberculosis Erdman day-20 7H9 medium (MTB), cell culture supernatant extract (INTPHSE), GC, AM, lipoarabinomannan (LAM), phosphatidylinositol mannoside (PIM), fast-growing mycobacterial lipomannan (LM), mycolyl-arabinogalactan-peptidoglycan complex (mAGP), and total lipid fraction (TLF).	bind
13849	1	4720	5	NULL	NULL	0	NULL	Hsp70	NULL		bind	NULL				DC	NULL	immature			NULL		0	NULL	NULL	NULL	gw60_immunity_17_3_353_s_40	12354387	(C) Maleylated BSA inhibits Hsp70 binding to immature DC.	bind
13850	2	4720	5	NULL	NULL	0	NULL	BSA	NULL	maleylated	inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_immunity_17_3_353_s_40	12354387	(C) Maleylated BSA inhibits Hsp70 binding to immature DC.	bind
11918	1	4720	6	NULL	NULL	NULL	NULL	Hsp70	GP		bind					DC	Cell	immature			NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_3_353_s_40	12354387	(C) Maleylated BSA inhibits Hsp70 binding to immature DC.	bind
11919	2	4720	6	NULL	NULL	NULL	NULL	BSA	OrganismPart	maleylated	inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_3_353_s_40	12354387	(C) Maleylated BSA inhibits Hsp70 binding to immature DC.	bind
13851	1	4721	5	NULL	NULL	0	NULL		NULL		bind	NULL		Kalirin domains		TrkA	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_5106_s_277	15923627	(C) Mapping of Kalirin domains that bind TrkA by a GST  pulldown assay.	bind
11920	1	4721	6	NULL	NULL	NULL	NULL				bind			Kalirin domains		TrkA	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_5106_s_277	15923627	(C) Mapping of Kalirin domains that bind TrkA by a GST  pulldown assay.	bind
13852	1	4724	5	NULL	NULL	0	NULL	Mdl1	NULL		bind	NULL				F1F0-ATP synthase	NULL		F0 moiety		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_37_38338_s_173	15247210	(C) Mdl1 binds to the F0 moiety of the F1F0-ATP synthase.	bind
11921	1	4724	6	NULL	NULL	NULL	NULL	Mdl1	GP		bind					F1F0-ATP synthase	GP		F0 moiety		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_37_38338_s_173	15247210	(C) Mdl1 binds to the F0 moiety of the F1F0-ATP synthase.	bind
13853	1	4725	5	10	NULL	0	NULL	p53			bind					Apaf-1				promoter	NULL	MEF	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_9_3492_s_119	16611991	(C) MEFs (p53+/+) and primary MEFs (p53+/+) were analyzed by ChIP for p53 binding to the  Apaf-1 gene promoter in the absence of stress.	bind
54483	2	4725	5	10	NULL	0	NULL	p53			bind					Apaf-1				promoter	NULL	primary MEF	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_9_3492_s_119	16611991	(C) MEFs (p53+/+) and primary MEFs (p53+/+) were analyzed by ChIP for p53 binding to the  Apaf-1 gene promoter in the absence of stress.	bind
11997	1	4725	6	NULL	NULL	NULL	NULL	p53	GP		bind					Apaf-1 	GP			promoter	NULL	MEF	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_9_3492_s_119	16611991	(C) MEFs (p53+/+) and primary MEFs (p53+/+) were analyzed by ChIP for p53 binding to the  Apaf-1 gene promoter in the absence of stress.	bind
11998	2	4725	6	NULL	NULL	NULL	NULL	p53	GP		bind					Apaf-1	GP			promoter	NULL	primary MEF	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_9_3492_s_119	16611991	(C) MEFs (p53+/+) and primary MEFs (p53+/+) were analyzed by ChIP for p53 binding to the  Apaf-1 gene promoter in the absence of stress.	bind
13854	1	4726	5	NULL	NULL	0	NULL	MIBP1	NULL		bind	NULL				SSTR-2	NULL			promoter	NULL	in vivo	0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3736_s_122	10207097	(C) MIBP1 binds to the SSTR-2 promoter in vivo.	bind
11999	1	4726	6	NULL	NULL	NULL	NULL	MIBP1	GP		bind					SSTR-2	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3736_s_122	10207097	(C) MIBP1 binds to the SSTR-2 promoter in vivo.	bind
13855	1	4727	5	NULL	NULL	0	NULL	MKP5	NULL		bind	NULL				JNK	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_19_8619_s_258	16166642	(c) MKP5 binding to JNK increases  in cells that were treated with JAMP siRNA.	bind
44571	2	4727	5	10	NULL	0	NULL	JAMP siRNA	NULL		increase	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_19_8619_s_258	16166642	(c) MKP5 binding to JNK increases  in cells that were treated with JAMP siRNA.	bind
12000	1	4727	6	NULL	NULL	NULL	NULL	MKP5	GP		bind					JNK	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8619_s_258	16166642	(c) MKP5 binding to JNK increases  in cells that were treated with JAMP siRNA.	bind
12001	2	4727	6	NULL	NULL	NULL	NULL	JAMP siRNA	NucleicAcid		increases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8619_s_258	16166642	(c) MKP5 binding to JNK increases  in cells that were treated with JAMP siRNA.	bind
13857	1	4728	5	10	NULL	0	NULL	MOD1			bind					CAF-1			p150 N-terminal domain		NULL		NULL	NULL	NULL	NULL	gw60_molcell_4_4_529_s_65	10549285	(C) MOD1 binds to CAF-1 primarily through the p150 N-terminal domain.	bind
12002	1	4728	6	NULL	NULL	NULL	NULL	MOD1	GP		bind					CAF-1	GP		p150 N-terminal domain		NULL		NULL	NULL	NULL	NULL	gw60_molcell_4_4_529_s_65	10549285	(C) MOD1 binds to CAF-1 primarily through the p150 N-terminal domain.	bind
13859	1	4729	5	10	NULL	0	NULL	 transcription factor		dimeric	bind					ERK2 dimer					NULL		NULL	NULL	NULL	NULL	gw60_cell_93_4_605_s_166	9604935	(C) Model of a dimeric transcription factor bound to an ERK2 dimer.	bind
15186	1	4729	6	NULL	NULL	NULL	NULL	transcription factor	GP	dimeric	bind					ERK2 dimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_93_4_605_s_166	9604935	(C) Model of a dimeric transcription factor bound to an ERK2 dimer.	bind
13860	1	4730	5	10	NULL	0	NULL	CopG			bind					DNA					NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_18_4943_s_40	12193609	(C) Model of CopG binding to its target DNA.	bind
12003	1	4730	6	NULL	NULL	NULL	NULL	CopG	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_18_4943_s_40	12193609	(C) Model of CopG binding to its target DNA.	bind
13861	1	4731	5	NULL	NULL	0	NULL	Mona	NULL		does not bind	NULL		SH2 domain		Gab3	NULL	phosphorylated	tyrosine		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_11_3744_s_160	11997510	(C) Mona SH2 domain does not bind to tyrosine phosphorylated Gab3.	bind
12004	1	4731	6	NULL	NULL	NULL	NULL	Mona	GP		does not bind			SH2 domain		Gab3	GP	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3744_s_160	11997510	(C) Mona SH2 domain does not bind to tyrosine phosphorylated Gab3.	bind
13862	1	4732	5	NULL	NULL	0	NULL	Six3	NULL	mouse	bind	NULL				Grg4	NULL				NULL	in mammalian cells	0	NULL	NULL	NULL	gw60_development_129_12_2835_s_153	12050133	(C) Mouse Six3 bound to Grg4 in mammalian cells.	bind
12005	1	4732	6	NULL	NULL	NULL	NULL	Six3	GP	mouse	bind					Grg4	GP				NULL	mammalian cells	NULL	NULL	NULL	NULL	gw60_development_129_12_2835_s_153	12050133	(C) Mouse Six3 bound to Grg4 in mammalian cells.	bind
13863	1	4734	5	NULL	NULL	0	NULL	Munc13-1	NULL		bind	NULL				RIM1	NULL		84 residue zinc finger domain		NULL		0	NULL	NULL	NULL	gw60_neuron_30_1_183_s_146	11343654	(C) Munc13-1 and Rab3A bind to the same 84 residue zinc finger domain of RIM1.	bind
13864	2	4734	5	NULL	NULL	0	NULL	Rab3A	NULL		bind	NULL				RIM1	NULL		84 residue zinc finger domain		NULL		0	NULL	NULL	NULL	gw60_neuron_30_1_183_s_146	11343654	(C) Munc13-1 and Rab3A bind to the same 84 residue zinc finger domain of RIM1.	bind
12006	1	4734	6	NULL	NULL	NULL	NULL	Munc13-1	GP		bind					RIM1	GP		84 residue zinc finger domain		NULL		NULL	NULL	NULL	NULL	gw60_neuron_30_1_183_s_146	11343654	(C) Munc13-1 and Rab3A bind to the same 84 residue zinc finger domain of RIM1.	bind
12007	2	4734	6	NULL	NULL	NULL	NULL	Rab3A	GP		bind					RIM1	GP		84 residue zinc finger domain		NULL		NULL	NULL	NULL	NULL	gw60_neuron_30_1_183_s_146	11343654	(C) Munc13-1 and Rab3A bind to the same 84 residue zinc finger domain of RIM1.	bind
13865	1	4735	5	NULL	NULL	0	NULL	RNF5	NULL	mutant	bind	NULL				paxillin	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_15_5331_s_134	12861019	(C) Mutant forms of RNF5 exhibit stronger binding to paxillin than wild-type RNF5.	bind
13866	2	4735	5	NULL	NULL	0	NULL	RNF5	NULL	wild-type	bind	NULL				paxillin	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_15_5331_s_134	12861019	(C) Mutant forms of RNF5 exhibit stronger binding to paxillin than wild-type RNF5.	bind
13867	3	4735	5	NULL	NULL	0	NULL	statement 1	NULL		is stronger than	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_15_5331_s_134	12861019	(C) Mutant forms of RNF5 exhibit stronger binding to paxillin than wild-type RNF5.	bind
12008	1	4735	6	NULL	NULL	NULL	NULL	RNF5	GP	wild type	bind					paxillin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_15_5331_s_134	12861019	(C) Mutant forms of RNF5 exhibit stronger binding to paxillin than wild-type RNF5.	bind
12009	2	4735	6	NULL	NULL	NULL	NULL	RNF5	GP	mutant	bind					paxillin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_15_5331_s_134	12861019	(C) Mutant forms of RNF5 exhibit stronger binding to paxillin than wild-type RNF5.	bind
12010	3	4735	6	NULL	NULL	NULL	NULL	statement 2	Process		is greater than					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_15_5331_s_134	12861019	(C) Mutant forms of RNF5 exhibit stronger binding to paxillin than wild-type RNF5.	bind
13868	1	4736	5	NULL	NULL	0	NULL	Tom22	NULL	mutant	alter	NULL		cytosolic domain		Tom40	NULL	oligomeric structure of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_9_5256_s_140	9710610	(C) Mutations in the cytosolic domain of Tom22 alter the oligomeric structure of Tom40.	bind
12011	1	4736	6	NULL	NULL	NULL	NULL	Tom22	GP	mutant	alter			cytosolic domain		Tom40	GP	oligomeric structure of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5256_s_140	9710610	(C) Mutations in the cytosolic domain of Tom22 alter the oligomeric structure of Tom40.	bind
13869	1	4737	5	NULL	NULL	0	NULL	Vg1RBP/Vera	NULL		bind	NULL				Vg1 LS	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_10_4669_s_242	15292452	(C) Mutations within E2 or R1 motifs do not affect binding of Vg1RBP/Vera  to the Vg1 LS and Xcat2 3'UTR.	bind
13870	2	4737	5	NULL	NULL	0	NULL	Vg1RBP/Vera	NULL		bind	NULL				Xcat2	NULL			3'UTR	NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_10_4669_s_242	15292452	(C) Mutations within E2 or R1 motifs do not affect binding of Vg1RBP/Vera  to the Vg1 LS and Xcat2 3'UTR.	bind
13871	3	4737	5	NULL	NULL	0	NULL		NULL	mutant	does not affect	NULL			E2 motif	statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_10_4669_s_242	15292452	(C) Mutations within E2 or R1 motifs do not affect binding of Vg1RBP/Vera  to the Vg1 LS and Xcat2 3'UTR.	bind
13872	4	4737	5	NULL	NULL	0	NULL		NULL	mutant	does not affect	NULL			R1 motif	statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_10_4669_s_242	15292452	(C) Mutations within E2 or R1 motifs do not affect binding of Vg1RBP/Vera  to the Vg1 LS and Xcat2 3'UTR.	bind
13873	5	4737	5	NULL	NULL	0	NULL	statement 3	NULL		is an alternative to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_10_4669_s_242	15292452	(C) Mutations within E2 or R1 motifs do not affect binding of Vg1RBP/Vera  to the Vg1 LS and Xcat2 3'UTR.	bind
13874	6	4737	5	NULL	NULL	0	NULL		NULL	mutant	does not affect	NULL			E2 motif	statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_10_4669_s_242	15292452	(C) Mutations within E2 or R1 motifs do not affect binding of Vg1RBP/Vera  to the Vg1 LS and Xcat2 3'UTR.	bind
13875	7	4737	5	NULL	NULL	0	NULL		NULL	mutant	does not affect	NULL			R1 motif	statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_10_4669_s_242	15292452	(C) Mutations within E2 or R1 motifs do not affect binding of Vg1RBP/Vera  to the Vg1 LS and Xcat2 3'UTR.	bind
13876	8	4737	5	NULL	NULL	0	NULL	statement 6	NULL		is an alternative to	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_10_4669_s_242	15292452	(C) Mutations within E2 or R1 motifs do not affect binding of Vg1RBP/Vera  to the Vg1 LS and Xcat2 3'UTR.	bind
12012	1	4737	6	NULL	NULL	NULL	NULL	Vg1RBP/Vera	GP		bind					Vg1	GP		LS		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_10_4669_s_242	15292452	(C) Mutations within E2 or R1 motifs do not affect binding of Vg1RBP/Vera  to the Vg1 LS and Xcat2 3'UTR.	bind
12013	2	4737	6	NULL	NULL	NULL	NULL	Vg1RBP/Vera	GP		bind					Xcat2	GP			3'UTR	NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_10_4669_s_242	15292452	(C) Mutations within E2 or R1 motifs do not affect binding of Vg1RBP/Vera  to the Vg1 LS and Xcat2 3'UTR.	bind
15187	3	4737	6	NULL	NULL	NULL	NULL			mutations of	do not affect			E2 motif		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_10_4669_s_242	15292452	(C) Mutations within E2 or R1 motifs do not affect binding of Vg1RBP/Vera  to the Vg1 LS and Xcat2 3'UTR.	bind
15188	4	4737	6	NULL	NULL	NULL	NULL			mutations of	do not affect			R1 motif		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_10_4669_s_242	15292452	(C) Mutations within E2 or R1 motifs do not affect binding of Vg1RBP/Vera  to the Vg1 LS and Xcat2 3'UTR.	bind
15189	5	4737	6	NULL	NULL	NULL	NULL			mutations of	do not affect			E2 motif		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_10_4669_s_242	15292452	(C) Mutations within E2 or R1 motifs do not affect binding of Vg1RBP/Vera  to the Vg1 LS and Xcat2 3'UTR.	bind
15190	6	4737	6	NULL	NULL	NULL	NULL			mutations of	do not affect			R1 motif		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_10_4669_s_242	15292452	(C) Mutations within E2 or R1 motifs do not affect binding of Vg1RBP/Vera  to the Vg1 LS and Xcat2 3'UTR.	bind
54491	7	4737	6	NULL	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_10_4669_s_242	15292452	(C) Mutations within E2 or R1 motifs do not affect binding of Vg1RBP/Vera  to the Vg1 LS and Xcat2 3'UTR.	bind
54492	8	4737	6	NULL	NULL	NULL	NULL	statement 5	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_10_4669_s_242	15292452	(C) Mutations within E2 or R1 motifs do not affect binding of Vg1RBP/Vera  to the Vg1 LS and Xcat2 3'UTR.	bind
13877	1	4738	5	NULL	NULL	0	NULL	Sp1	NULL		bind	NULL				probe B	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_3_2098_s_209	10022897	(C) Mutual exclusive binding of Sp1 and NF-kappaB p50 to probe B.	bind
13878	2	4738	5	NULL	NULL	0	NULL	NF-kappaB p50	NULL		bind	NULL				probe B	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_3_2098_s_209	10022897	(C) Mutual exclusive binding of Sp1 and NF-kappaB p50 to probe B.	bind
13879	3	4738	5	NULL	NULL	0	NULL	statement 1	NULL		mutually exclusive to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_3_2098_s_209	10022897	(C) Mutual exclusive binding of Sp1 and NF-kappaB p50 to probe B.	bind
12015	1	4738	6	NULL	NULL	NULL	NULL	Sp1	GP		bind					probe B					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_2098_s_209	10022897	(C) Mutual exclusive binding of Sp1 and NF-kappaB p50 to probe B.	bind
12016	2	4738	6	NULL	NULL	NULL	NULL	NF-kappaB p50	GP		bind					probe B					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_2098_s_209	10022897	(C) Mutual exclusive binding of Sp1 and NF-kappaB p50 to probe B.	bind
12017	3	4738	6	NULL	NULL	NULL	NULL	statement 1	Process		is independent of					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_2098_s_209	10022897	(C) Mutual exclusive binding of Sp1 and NF-kappaB p50 to probe B.	bind
13880	1	4739	5	NULL	NULL	0	NULL	Myricetin	NULL		bind	NULL				PI3K	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_6_4_909_s_221	11090628	(C) Myricetin binding to PI3K  as compared with quercetin binding to PI3K .	bind
13881	2	4739	5	NULL	NULL	0	NULL	quercetin	NULL		bind	NULL				PI3K	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_6_4_909_s_221	11090628	(C) Myricetin binding to PI3K  as compared with quercetin binding to PI3K .	bind
12018	1	4739	6	NULL	NULL	NULL	NULL	Myricetin	GP		bind					PI3K	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_4_909_s_221	11090628	(C) Myricetin binding to PI3K  as compared with quercetin binding to PI3K .	bind
12019	2	4739	6	NULL	NULL	NULL	NULL	quercetin	GP		bind					PI3K	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_4_909_s_221	11090628	(C) Myricetin binding to PI3K  as compared with quercetin binding to PI3K .	bind
13882	1	4740	5	NULL	NULL	0	NULL	AP-2 protein	NULL		does not bind	NULL		N-terminally deleted		RB	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_7_3647_s_227	9632747	(C) N-terminally deleted AP-2 protein does not bind to RB.	bind
12020	1	4740	6	NULL	NULL	NULL	NULL	AP-2 protein	GP		does not bind			N-terminally deleted		RB	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_3647_s_227	9632747	(C) N-terminally deleted AP-2 protein does not bind to RB.	bind
13883	1	4741	5	NULL	NULL	0	NULL	Nef	NULL		bind	NULL				PAK1	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_molcellbiol_20_7_2619_s_111	10713183	(C) Nef binds to PAK1 in vitro.	bind
12021	1	4741	6	NULL	NULL	NULL	NULL	Nef	GP		bind					PAK1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_7_2619_s_111	10713183	(C) Nef binds to PAK1 in vitro.	bind
13884	1	4742	5	NULL	NULL	0	NULL	Neurexin	NULL		bind	NULL				neuroligin	NULL	mutants of			NULL		0	NULL	NULL	NULL	gw60_cell_101_6_657_s_190	10892652	(C) Neurexin binding of neuroligin mutants.	bind
12022	1	4742	6	NULL	NULL	NULL	NULL	Neurexin	GP		bind					neuroligin	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_cell_101_6_657_s_190	10892652	(C) Neurexin binding of neuroligin mutants.	bind
13885	1	4743	5	NULL	NULL	0	NULL	aconitase	NULL	newly translated in E. coli	bind	NULL				GroEL	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_107_2_235_s_48	11672530	(c) Newly translated aconitase in  E. coli is  bound to GroEL and released from it  in the presence but not absence of  GroES.	bind
13886	2	4743	5	NULL	NULL	0	NULL	aconitase	NULL	newly translated in E. coli	is released from	NULL				GroEL	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_107_2_235_s_48	11672530	(c) Newly translated aconitase in  E. coli is  bound to GroEL and released from it  in the presence but not absence of  GroES.	bind
13887	3	4743	5	NULL	NULL	0	NULL	statement 2	NULL		in the presence of	NULL	only			GroES	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_107_2_235_s_48	11672530	(c) Newly translated aconitase in  E. coli is  bound to GroEL and released from it  in the presence but not absence of  GroES.	bind
12023	1	4743	6	NULL	NULL	NULL	NULL	aconitase	GP	newly translated;; E.coli	bind					GroEL	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_235_s_48	11672530	(c) Newly translated aconitase in  E. coli is  bound to GroEL and released from it  in the presence but not absence of  GroES.	bind
12024	2	4743	6	NULL	NULL	NULL	NULL	aconitase	GP	newly translated;; E.coli	released from					GroEL	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_235_s_48	11672530	(c) Newly translated aconitase in  E. coli is  bound to GroEL and released from it  in the presence but not absence of  GroES.	bind
12025	3	4743	6	NULL	NULL	NULL	NULL	statement 2	Process		occurs in presence of					GroES	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_235_s_48	11672530	(c) Newly translated aconitase in  E. coli is  bound to GroEL and released from it  in the presence but not absence of  GroES.	bind
13888	1	4744	5	NULL	NULL	0	NULL	class II UNC-86 	NULL	mutant	bind	NULL	very weakly			CS1 oligonucleotide	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_13_4806_s_161	10848606	(C) No or very weak binding of class II and III UNC-86 mutants to the CS1 oligonucleotide could be detected at the protein concentrations used.	bind
13889	2	4744	5	NULL	NULL	0	NULL	class III UNC-86	NULL	mutant	bind	NULL	very weakly			CS1 oligonucleotide	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_13_4806_s_161	10848606	(C) No or very weak binding of class II and III UNC-86 mutants to the CS1 oligonucleotide could be detected at the protein concentrations used.	bind
54493	3	4744	5	10	NULL	0	NULL	class II UNC-86		mutant	does not bind					CS1 oligonucleotide					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4806_s_161	10848606	(C) No or very weak binding of class II and III UNC-86 mutants to the CS1 oligonucleotide could be detected at the protein concentrations used.	bind
54494	4	4744	5	10	NULL	0	NULL	class III UNC-86		mutant	does not bind					CS1 oligonucleotide					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_13_4806_s_161	10848606	(C) No or very weak binding of class II and III UNC-86 mutants to the CS1 oligonucleotide could be detected at the protein concentrations used.	bind
54495	5	4744	5	10	NULL	0	NULL	statement 1			is an alternative to					statement 3					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_13_4806_s_161	10848606	(C) No or very weak binding of class II and III UNC-86 mutants to the CS1 oligonucleotide could be detected at the protein concentrations used.	bind
54496	6	4744	5	10	NULL	0	NULL	statement 2			is an alternative to					statement 4					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_13_4806_s_161	10848606	(C) No or very weak binding of class II and III UNC-86 mutants to the CS1 oligonucleotide could be detected at the protein concentrations used.	bind
12026	1	4744	6	NULL	NULL	NULL	NULL	class II UNC-86	GP	mutant	bind		weakly			CS1 oligonucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4806_s_161	10848606	(C) No or very weak binding of class II and III UNC-86 mutants to the CS1 oligonucleotide could be detected at the protein concentrations used.	bind
12027	2	4744	6	NULL	NULL	NULL	NULL	class III UNC-86	GP	mutant	bind		weakly			CS1 oligonucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4806_s_161	10848606	(C) No or very weak binding of class II and III UNC-86 mutants to the CS1 oligonucleotide could be detected at the protein concentrations used.	bind
12028	3	4744	6	NULL	NULL	NULL	NULL	class II UNC-86	GP	mutant	does not bind					CS1 oligonucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4806_s_161	10848606	(C) No or very weak binding of class II and III UNC-86 mutants to the CS1 oligonucleotide could be detected at the protein concentrations used.	bind
12029	4	4744	6	NULL	NULL	NULL	NULL	class III UNC-86	GP	mutant	does not bind					CS1 oligonucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4806_s_161	10848606	(C) No or very weak binding of class II and III UNC-86 mutants to the CS1 oligonucleotide could be detected at the protein concentrations used.	bind
12030	5	4744	6	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4806_s_161	10848606	(C) No or very weak binding of class II and III UNC-86 mutants to the CS1 oligonucleotide could be detected at the protein concentrations used.	bind
12031	6	4744	6	NULL	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4806_s_161	10848606	(C) No or very weak binding of class II and III UNC-86 mutants to the CS1 oligonucleotide could be detected at the protein concentrations used.	bind
13890	1	4745	5	NULL	NULL	0	NULL	NSF	NULL		does not bind	NULL	alone			PICK1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuron_34_1_53_s_63	11931741	(C) NSF does not bind PICK1 alone.	bind
12032	1	4745	6	NULL	NULL	NULL	NULL	NSF	GP		does not bind		alone			PICK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_34_1_53_s_63	11931741	(C) NSF does not bind PICK1 alone.	bind
13891	3	4746	5	10	NULL	0	NULL	statement 1			is not increased by					HNF3betaloxP/loxP; Alb					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_14_5175_s_161	10866673	(C) Nuclear binding activities of HNF3alpha and HNF3gamma are not increased in HNF3betaloxP/loxP; Alb.	bind
13892	4	4746	5	10	NULL	0	NULL	statement 2			is not increased by					HNF3betaloxP/loxP; Alb					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_14_5175_s_161	10866673	(C) Nuclear binding activities of HNF3alpha and HNF3gamma are not increased in HNF3betaloxP/loxP; Alb.	bind
54497	1	4746	5	10	NULL	0	NULL	HNF3alpha 			possess					 Nuclear binding activity					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_14_5175_s_161	10866673	(C) Nuclear binding activities of HNF3alpha and HNF3gamma are not increased in HNF3betaloxP/loxP; Alb.	bind
54498	2	4746	5	10	NULL	0	NULL	HNF3gamma			possess					Nuclear binding activity					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_14_5175_s_161	10866673	(C) Nuclear binding activities of HNF3alpha and HNF3gamma are not increased in HNF3betaloxP/loxP; Alb.	bind
15191	1	4746	6	NULL	NULL	NULL	NULL	HNF3alpha	GP		possess					Nuclear binding activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_14_5175_s_161	10866673	(C) Nuclear binding activities of HNF3alpha and HNF3gamma are not increased in HNF3betaloxP/loxP; Alb.	bind
15192	2	4746	6	NULL	NULL	NULL	NULL	HNF3gamma	GP		possess					Nuclear binding activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_14_5175_s_161	10866673	(C) Nuclear binding activities of HNF3alpha and HNF3gamma are not increased in HNF3betaloxP/loxP; Alb.	bind
41570	3	4746	6	NULL	NULL	NULL	NULL	statement 1	Process		is not increased by					HNF3betaloxP/loxP; Alb	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_14_5175_s_161	10866673	(C) Nuclear binding activities of HNF3alpha and HNF3gamma are not increased in HNF3betaloxP/loxP; Alb.	bind
41571	4	4746	6	NULL	NULL	NULL	NULL	statement 2	Process		is not increased by					HNF3betaloxP/loxP; Alb	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_14_5175_s_161	10866673	(C) Nuclear binding activities of HNF3alpha and HNF3gamma are not increased in HNF3betaloxP/loxP; Alb.	bind
13893	1	4749	5	NULL	NULL	0	NULL	Optineurin	NULL		bind	NULL				myosin VI	NULL	purified	tail		NULL		0	NULL	NULL	NULL	gw70_cellbiol_169_2_285_s_63	15837803	(C) Optineurin binds to purified  myosin VI tail.	bind
12033	1	4749	6	NULL	NULL	NULL	NULL	optineurin	GP		bind					myosin VI 	GP	purified	tail		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_169_2_285_s_63	15837803	(C) Optineurin binds to purified  myosin VI tail.	bind
13894	1	4750	5	NULL	NULL	0	NULL	UBF	NULL		bind	NULL				rRNA gene	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_7_2539_s_178	15767661	(C) Overexpression of TIP5 impairs binding  of UBF to the rRNA gene promoter.	bind
13895	2	4750	5	NULL	NULL	0	NULL	TIP5	NULL	overexpression of	impairs	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_7_2539_s_178	15767661	(C) Overexpression of TIP5 impairs binding  of UBF to the rRNA gene promoter.	bind
12034	1	4750	6	NULL	NULL	NULL	NULL	UBF	GP		bind					rRNA 	NucleicAcid			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_7_2539_s_178	15767661	(C) Overexpression of TIP5 impairs binding  of UBF to the rRNA gene promoter.	bind
12035	2	4750	6	NULL	NULL	NULL	NULL	TIP5 	GP	overexpression of	impairs					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_7_2539_s_178	15767661	(C) Overexpression of TIP5 impairs binding  of UBF to the rRNA gene promoter.	bind
13896	1	4755	5	NULL	NULL	0	NULL	OxyR	NULL		bind	NULL				ahpC	NULL	M. marinum		promoter region	NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_7_2674_s_134	16547055	(C) OxyR binds to the  M. marinum ahpC promoter region.	bind
12036	1	4755	6	NULL	NULL	NULL	NULL	OxyR	GP		bind					ahpC	GP	M. marinum		promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_7_2674_s_134	16547055	(C) OxyR binds to the  M. marinum ahpC promoter region.	bind
13897	1	4756	5	10	NULL	0	NULL	p27		phosphorylated	bind			serine 10		GRB2					NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_11_3735_s_293	12748278	(C) p27 bound to GRB2 is phosphorylated on serine  10.	bind
12037	1	4756	6	NULL	NULL	NULL	NULL	p27	GP	phosphorylated	bind			serine 10		GRB2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_11_3735_s_293	12748278	(C) p27 bound to GRB2 is phosphorylated on serine  10.	bind
13899	1	4758	5	NULL	NULL	0	NULL	p53	NULL		bind	NULL	specifically				NULL			p53RE-1	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5602_s_205	10891498	(C) p53 binds specifically to both p53RE-1 and p53RE-2 in vitro.	bind
13900	2	4758	5	NULL	NULL	0	NULL	p53	NULL		bind	NULL	specifically				NULL			p53RE-2	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5602_s_205	10891498	(C) p53 binds specifically to both p53RE-1 and p53RE-2 in vitro.	bind
12038	1	4758	6	NULL	NULL	NULL	NULL	p53	GP		bind		specifically							p53RE-1	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5602_s_205	10891498	(C) p53 binds specifically to both p53RE-1 and p53RE-2 in vitro.	bind
12039	2	4758	6	NULL	NULL	NULL	NULL	p53	GP		bind		specifically							p53RE-2	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5602_s_205	10891498	(C) p53 binds specifically to both p53RE-1 and p53RE-2 in vitro.	bind
13901	1	4759	5	NULL	NULL	0	NULL	CREB	NULL		bind	NULL				CBP	NULL		KIX domain		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_13_4849_s_96	10848610	(C) p53 does not enhance the binding of CREB to the KIX domain of CBP.	bind
13902	2	4759	5	NULL	NULL	0	NULL	p53	NULL		does not enhance	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_13_4849_s_96	10848610	(C) p53 does not enhance the binding of CREB to the KIX domain of CBP.	bind
12040	1	4759	6	NULL	NULL	NULL	NULL	CREB	GP		bind					CBP	GP		KIX domain		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4849_s_96	10848610	(C) p53 does not enhance the binding of CREB to the KIX domain of CBP.	bind
12041	2	4759	6	NULL	NULL	NULL	NULL	p53	GP		does not enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4849_s_96	10848610	(C) p53 does not enhance the binding of CREB to the KIX domain of CBP.	bind
13903	1	4760	5	NULL	NULL	0	NULL	SRC-1	NULL		bind	NULL				Nur77	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_7_2593_s_271	15024051	(C) p65  interfered with the binding of the coactivator SRC-1 to Nur77 in GST pull-down assays.	bind
13904	2	4760	5	NULL	NULL	0	NULL	p65	NULL		interferes with	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_7_2593_s_271	15024051	(C) p65  interfered with the binding of the coactivator SRC-1 to Nur77 in GST pull-down assays.	bind
54505	3	4760	5	10	NULL	0	NULL	SRC-1			is a type of					coactivator					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_7_2593_s_271	15024051	(C) p65  interfered with the binding of the coactivator SRC-1 to Nur77 in GST pull-down assays.	bind
12042	1	4760	6	NULL	NULL	NULL	NULL	SRC-1	GP		bind					Nur77	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_7_2593_s_271	15024051	(C) p65  interfered with the binding of the coactivator SRC-1 to Nur77 in GST pull-down assays.	bind
12043	2	4760	6	NULL	NULL	NULL	NULL	p65	GP		interferes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_7_2593_s_271	15024051	(C) p65  interfered with the binding of the coactivator SRC-1 to Nur77 in GST pull-down assays.	bind
41575	3	4760	6	NULL	NULL	NULL	NULL	SRC-1	GP		is a type of					coactivator	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_7_2593_s_271	15024051	(C) p65  interfered with the binding of the coactivator SRC-1 to Nur77 in GST pull-down assays.	bind
13905	1	4761	5	NULL	NULL	0	NULL	p73	NULL		bind	NULL				p73	NULL		Ndelta		NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_8_3536_s_329	15060172	(C) p73 binds to p73Ndelta but not to p73 lacking the putative tetramerization domain.	bind
13906	2	4761	5	10	NULL	0	NULL	p73			does not bind					p73		lacking;;putative	 tetramerization domain		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_8_3536_s_329	15060172	(C) p73 binds to p73Ndelta but not to p73 lacking the putative tetramerization domain.	bind
12044	1	4761	6	NULL	NULL	0	NULL	p73	NULL		bind	NULL				p73	NULL		Ndelta		NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_8_3536_s_329	15060172	(C) p73 binds to p73Ndelta but not to p73 lacking the putative tetramerization domain.	bind
12045	2	4761	6	NULL	NULL	0	NULL	p73	NULL		does not bind	NULL				p73	NULL	lacking;; putative	tetramerization domain		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_8_3536_s_329	15060172	(C) p73 binds to p73Ndelta but not to p73 lacking the putative tetramerization domain.	bind
13907	1	4762	5	NULL	NULL	0	NULL	PAG3	NULL		bind	NULL				paxillin isoforms	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_4_1315_s_142	10749932	(C) PAG3 binding to paxillin isoforms.	bind
12046	1	4762	6	NULL	NULL	NULL	NULL	PAG3	GP		bind					paxillin isoforms	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_4_1315_s_142	10749932	(C) PAG3 binding to paxillin isoforms.	bind
13908	1	4763	5	NULL	NULL	0	NULL	PAK	NULL		bind	NULL				PIX-GIT1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_11_3906_s_247	10805734	(C) PAK binding to PIX-GIT1 is negatively regulated by kinase activation.	bind
13909	2	4763	5	10	NULL	0	NULL	statement 1			regulated by		negatively			kinase		activation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_11_3906_s_247	10805734	(C) PAK binding to PIX-GIT1 is negatively regulated by kinase activation.	bind
12047	1	4763	6	NULL	NULL	NULL	NULL	PAK	GP		bind					PIX-GIT1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_11_3906_s_247	10805734	(C) PAK binding to PIX-GIT1 is negatively regulated by kinase activation.	bind
12048	2	4763	6	NULL	NULL	NULL	NULL	statement 1	Process		regulated by		negatively 			kinase	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_11_3906_s_247	10805734	(C) PAK binding to PIX-GIT1 is negatively regulated by kinase activation.	bind
13910	1	4764	5	NULL	NULL	0	NULL	Pax1	NULL		bind	NULL				oligonucleotide B4	NULL				NULL		0	NULL	NULL	NULL	gw70_development_130_3_473_s_126	12490554	(C) Pax1  binds to oligonucleotide B4.	bind
12049	1	4764	6	NULL	NULL	NULL	NULL	Pax1	GP		bind					oligonucleotide B4	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_development_130_3_473_s_126	12490554	(C) Pax1  binds to oligonucleotide B4.	bind
13911	1	4766	5	NULL	NULL	0	NULL		NULL		bind	NULL		N		GST-RDGCcat	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_32_6_1097_s_227	11754840	(C) Percent of N or NI12E bound to GST-RDGCcat in the presence of Ca2+/aM (from [B]).	bind
13912	2	4766	5	NULL	NULL	0	NULL		NULL		bind	NULL		NI12E		GST-RDGCcat 	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_32_6_1097_s_227	11754840	(C) Percent of N or NI12E bound to GST-RDGCcat in the presence of Ca2+/aM (from [B]).	bind
15587	3	4766	5	NULL	NULL	0	NULL	statement 1	NULL		in the presence of	NULL				Ca2+	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_32_6_1097_s_227	11754840	(C) Percent of N or NI12E bound to GST-RDGCcat in the presence of Ca2+/aM (from [B]).	bind
15588	4	4766	5	NULL	NULL	0	NULL	statement 2	NULL		in the presence of	NULL				Ca2+	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_32_6_1097_s_227	11754840	(C) Percent of N or NI12E bound to GST-RDGCcat in the presence of Ca2+/aM (from [B]).	bind
12299	1	4766	6	NULL	NULL	NULL	NULL				bind			NI12E		GST-RDGCcat	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_6_1097_s_227	11754840	(C) Percent of N or NI12E bound to GST-RDGCcat in the presence of Ca2+/aM (from [B]).	bind
12300	2	4766	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs in presence of					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_6_1097_s_227	11754840	(C) Percent of N or NI12E bound to GST-RDGCcat in the presence of Ca2+/aM (from [B]).	bind
16241	3	4766	6	NULL	NULL	NULL	NULL				bind			N terminal domain		GST-RDGCcat	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_6_1097_s_227	11754840	(C) Percent of N or NI12E bound to GST-RDGCcat in the presence of Ca2+/aM (from [B]).	bind
16242	4	4766	6	NULL	NULL	NULL	NULL	statement 2	Process		occurs in presence of					Ca+2	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_6_1097_s_227	11754840	(C) Percent of N or NI12E bound to GST-RDGCcat in the presence of Ca2+/aM (from [B]).	bind
13913	1	4767	5	NULL	NULL	0	NULL	PEX7	NULL		bind	NULL	inefficient			pex5-1	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_2_573_s_228	15548601	(C) PEX7 binding  with pex5-1 is inefficient, resulting in decreased PTS2 protein import and IBA resistance.	bind
13914	2	4767	5	NULL	NULL	0	NULL	statement 1	NULL		results in	NULL				PTS2 protein	NULL	decreased import of			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_2_573_s_228	15548601	(C) PEX7 binding  with pex5-1 is inefficient, resulting in decreased PTS2 protein import and IBA resistance.	bind
13915	3	4767	5	NULL	NULL	0	NULL	statement 1	NULL		results in	NULL				IBA resistance	NULL	decreased			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_2_573_s_228	15548601	(C) PEX7 binding  with pex5-1 is inefficient, resulting in decreased PTS2 protein import and IBA resistance.	bind
12050	1	4767	6	NULL	NULL	NULL	NULL	PEX7	GP		bind		inefficiently			pex5-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_2_573_s_228	15548601	(C) PEX7 binding  with pex5-1 is inefficient, resulting in decreased PTS2 protein import and IBA resistance.	bind
12051	2	4767	6	NULL	NULL	NULL	NULL	statement 1	Process		leads to					PTS2 protein 	GP	decreased import of			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_2_573_s_228	15548601	(C) PEX7 binding  with pex5-1 is inefficient, resulting in decreased PTS2 protein import and IBA resistance.	bind
12052	3	4767	6	NULL	NULL	NULL	NULL	statement 1	Process		leads to					IBA 	Chemical	resistance of			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_2_573_s_228	15548601	(C) PEX7 binding  with pex5-1 is inefficient, resulting in decreased PTS2 protein import and IBA resistance.	bind
14579	1	4768	5	10	NULL	0	NULL	EGFR		 blocking function of	diminishes					Ras/MAPK		active			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_1_103_s_65	12370245	(c) Pharmacologic blockade of EGFR function diminishes active Ras/MAPK, Gab1 tyrosine phosphorylation, and binding to SHP-2.	bind
14580	2	4768	5	10	NULL	0	NULL	EGFR		blocking  function of	diminishes					Gab1		phosphorylation	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_1_103_s_65	12370245	(c) Pharmacologic blockade of EGFR function diminishes active Ras/MAPK, Gab1 tyrosine phosphorylation, and binding to SHP-2.	bind
14581	3	4768	5	NULL	NULL	0	NULL	Gab1	NULL		bind	NULL				SHP-2	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_159_1_103_s_65	12370245	(c) Pharmacologic blockade of EGFR function diminishes active Ras/MAPK, Gab1 tyrosine phosphorylation, and binding to SHP-2.	bind
14582	4	4768	5	10	NULL	0	NULL	EGFR		blocking function of	diminishes					statement 3					NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_1_103_s_65	12370245	(c) Pharmacologic blockade of EGFR function diminishes active Ras/MAPK, Gab1 tyrosine phosphorylation, and binding to SHP-2.	bind
12053	1	4768	6	NULL	NULL	NULL	NULL	Gab1	GP		bind					SHP-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_1_103_s_65	12370245	(c) Pharmacologic blockade of EGFR function diminishes active Ras/MAPK, Gab1 tyrosine phosphorylation, and binding to SHP-2.	bind
12054	2	4768	6	NULL	NULL	NULL	NULL	EGFR 	GP	blocking function of	diminishes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_1_103_s_65	12370245	(c) Pharmacologic blockade of EGFR function diminishes active Ras/MAPK, Gab1 tyrosine phosphorylation, and binding to SHP-2.	bind
12055	3	4768	6	NULL	NULL	NULL	NULL	Gab1	GP		is phosphorylated on								tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_1_103_s_65	12370245	(c) Pharmacologic blockade of EGFR function diminishes active Ras/MAPK, Gab1 tyrosine phosphorylation, and binding to SHP-2.	bind
12056	4	4768	6	NULL	NULL	NULL	NULL	EGFR	GP	blocking function of	diminishes					Ras/MAPK	GP	active			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_1_103_s_65	12370245	(c) Pharmacologic blockade of EGFR function diminishes active Ras/MAPK, Gab1 tyrosine phosphorylation, and binding to SHP-2.	bind
12452	5	4768	6	NULL	NULL	NULL	NULL	EGFR	GP	blocking function of	diminishes					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_1_103_s_65	12370245	(c) Pharmacologic blockade of EGFR function diminishes active Ras/MAPK, Gab1 tyrosine phosphorylation, and binding to SHP-2.	bind
13916	1	4769	5	NULL	NULL	0	NULL	PhoP P	NULL		bind	NULL				phoB-PS	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_15_5166_s_209	16030210	(C) PhoP P binds to the  phoB-PS promoter independent of the downstream direct repeats.	bind
13917	2	4769	5	NULL	NULL	0	NULL	statement 1	NULL		is independent of	NULL					NULL	downstream		direct repeats	NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_15_5166_s_209	16030210	(C) PhoP P binds to the  phoB-PS promoter independent of the downstream direct repeats.	bind
12057	1	4769	6	NULL	NULL	NULL	NULL	PhoP P 	GP		bind					phoB-PS	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_187_15_5166_s_209	16030210	(C) PhoP P binds to the  phoB-PS promoter independent of the downstream direct repeats.	bind
12058	2	4769	6	NULL	NULL	NULL	NULL	statement 1	Process		is independent of							downstream		direct repeats	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_187_15_5166_s_209	16030210	(C) PhoP P binds to the  phoB-PS promoter independent of the downstream direct repeats.	bind
13918	1	4770	5	NULL	NULL	0	NULL	DnaB	NULL	E. coli	bind	NULL				RTP	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_87_5_881_s_130	8945515	(C) Phosphorimager analyses  of the autoradiograms shown in (B); note that the mutations E30K and Y33N  have caused significant reduction in the binding of E. coli DnaB to the  RTP matrices.	bind
13919	2	4770	5	NULL	NULL	0	NULL		NULL	mutant	reduce	NULL	significantly	E30K		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_87_5_881_s_130	8945515	(C) Phosphorimager analyses  of the autoradiograms shown in (B); note that the mutations E30K and Y33N  have caused significant reduction in the binding of E. coli DnaB to the  RTP matrices.	bind
13920	3	4770	5	NULL	NULL	0	NULL		NULL	mutant	reduce	NULL	significantly	Y33N		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_87_5_881_s_130	8945515	(C) Phosphorimager analyses  of the autoradiograms shown in (B); note that the mutations E30K and Y33N  have caused significant reduction in the binding of E. coli DnaB to the  RTP matrices.	bind
12059	1	4770	6	NULL	NULL	NULL	NULL	DnaB	GP	E.coli	bind					RTP matrices	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_87_5_881_s_130	8945515	(C) Phosphorimager analyses  of the autoradiograms shown in (B); note that the mutations E30K and Y33N  have caused significant reduction in the binding of E. coli DnaB to the  RTP matrices.	bind
12060	2	4770	6	NULL	NULL	NULL	NULL			mutant	causes		significant	E30K		statement 1	Process	reduction in			NULL		NULL	NULL	NULL	NULL	gw60_cell_87_5_881_s_130	8945515	(C) Phosphorimager analyses  of the autoradiograms shown in (B); note that the mutations E30K and Y33N  have caused significant reduction in the binding of E. coli DnaB to the  RTP matrices.	bind
12061	3	4770	6	NULL	NULL	NULL	NULL			mutant	causes		significant	Y33N		statement 1	Process	reduction in			NULL		NULL	NULL	NULL	NULL	gw60_cell_87_5_881_s_130	8945515	(C) Phosphorimager analyses  of the autoradiograms shown in (B); note that the mutations E30K and Y33N  have caused significant reduction in the binding of E. coli DnaB to the  RTP matrices.	bind
13921	1	4771	5	NULL	NULL	0	NULL	PIP2	NULL		bind	NULL				syt I/IX constructs	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_162_2_199_s_211	12860971	(C) PIP2-binding activity of the indicated syt I/IX constructs was assayed as described in the legend to  Fig. 2 A. (D) PIP2 binding is correlated with inhibition of secretion.	bind
12062	1	4771	6	NULL	NULL	NULL	NULL	syt I/IX constructs			bind					PIP2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_162_2_199_s_211	12860971	(C) PIP2-binding activity of the indicated syt I/IX constructs was assayed as described in the legend to  Fig. 2 A. (D) PIP2 binding is correlated with inhibition of secretion.	bind
13922	1	4772	5	NULL	NULL	0	NULL	SRP	NULL		bind	NULL				bt-SR	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_162_4_575_s_173	12913112	(C) Plots of kon for SRP binding to bt-SR in the presence (solid symbols) or absence (open symbols)  of 25 muM GTP.	bind
12063	1	4772	6	NULL	NULL	NULL	NULL	SRP	GP		bind					bt-SR	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_162_4_575_s_173	12913112	(C) Plots of kon for SRP binding to bt-SR in the presence (solid symbols) or absence (open symbols)  of 25 muM GTP.	bind
13923	1	4774	5	NULL	NULL	0	NULL	p53	NULL	wild-type	bind	NULL				DNA	NULL	biotinylated target			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_7168_s_203	10490652	(C) PMA stimulates wild-type p53 binding to biotinylated target DNA.	bind
13924	2	4774	5	NULL	NULL	0	NULL	PMA	NULL		stimulate	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_10_7168_s_203	10490652	(C) PMA stimulates wild-type p53 binding to biotinylated target DNA.	bind
12064	1	4774	6	NULL	NULL	NULL	NULL	p53	GP	wild type	bind					target DNA	NucleicAcid	biotinylated			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_7168_s_203	10490652	(C) PMA stimulates wild-type p53 binding to biotinylated target DNA.	bind
12065	2	4774	6	NULL	NULL	NULL	NULL	PMA	Chemical		stimulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_7168_s_203	10490652	(C) PMA stimulates wild-type p53 binding to biotinylated target DNA.	bind
13925	1	4775	5	NULL	NULL	0	NULL	Poly(ADP-ribose)	NULL		bind	NULL				hTRF2	NULL		myb domain		NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_4_1595_s_240	14749375	(C) Poly(ADP-ribose) binds  to the myb domain of hTRF2.	bind
12066	1	4775	6	NULL	NULL	NULL	NULL	Poly (ADP-ribose)	Chemical		bind					hTRF2	GP		myb domain		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_4_1595_s_240	14749375	(C) Poly(ADP-ribose) binds  to the myb domain of hTRF2.	bind
13926	1	4776	5	NULL	NULL	0	NULL	cdk4	NULL		bind	NULL				p16	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_1_3_421_s_189	9660926	(C) Positive control for the effect of R24C mutation on the binding of cdk4 to p16.	bind
12067	1	4776	6	NULL	NULL	NULL	NULL	cdk4	GP		bind					p16	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_3_421_s_189	9660926	(C) Positive control for the effect of R24C mutation on the binding of cdk4 to p16.	bind
13927	1	4777	5	NULL	NULL	0	NULL	pp32	NULL		bind	NULL				TAF-I	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_cell_104_1_119_s_128	11163245	(C) pp32 binds to TAF-I , and Set/TAF-Ibeta in vitro.	bind
13928	2	4777	5	NULL	NULL	0	NULL	pp32	NULL		bind	NULL				Set/TAF-Ibeta	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_cell_104_1_119_s_128	11163245	(C) pp32 binds to TAF-I , and Set/TAF-Ibeta in vitro.	bind
12068	1	4777	6	NULL	NULL	NULL	NULL	pp32	GP		bind					TAF-I	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_cell_104_1_119_s_128	11163245	(C) pp32 binds to TAF-I , and Set/TAF-Ibeta in vitro.	bind
12069	2	4777	6	NULL	NULL	NULL	NULL	pp32	GP		bind					Set/TAF-Ibeta	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_cell_104_1_119_s_128	11163245	(C) pp32 binds to TAF-I , and Set/TAF-Ibeta in vitro.	bind
13930	1	4778	5	NULL	NULL	0	NULL	pRb	NULL		bind	NULL				E2F4	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_6_3_729_s_142	11030352	(C) pRb binds to E2F4 following the expression of p16INK4a.	bind
13931	2	4778	5	NULL	NULL	0	NULL	p16INK4a	NULL	expression of	leads to	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_6_3_729_s_142	11030352	(C) pRb binds to E2F4 following the expression of p16INK4a.	bind
12070	1	4778	6	NULL	NULL	NULL	NULL	pRb	GP		bind					E2F4	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_3_729_s_142	11030352	(C) pRb binds to E2F4 following the expression of p16INK4a.	bind
12071	2	4778	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs following					p16INK4a	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_3_729_s_142	11030352	(C) pRb binds to E2F4 following the expression of p16INK4a.	bind
14583	1	4779	5	10	NULL	0	NULL	Prohibitin			bind					HP1gamma			chromodomain		NULL	MCF-7 cell lysates	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4161_s_141	16705168	(C) Prohibitin  in the MCF-7 cell lysates binds to the chromodomain and chromoshadow domain of HP1gamma while Rb binds only to the chromoshadow domain.	bind
14584	2	4779	5	10	NULL	0	NULL	Prohibitin			bind					HP1gamma			chromoshadow domain		NULL	MCF-7 cell lysates	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4161_s_141	16705168	(C) Prohibitin  in the MCF-7 cell lysates binds to the chromodomain and chromoshadow domain of HP1gamma while Rb binds only to the chromoshadow domain.	bind
14585	3	4779	5	10	NULL	0	NULL	Rb			bind		only			HP1gamma			chromoshadow domain		NULL	MCF-7 cell lysates	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4161_s_141	16705168	(C) Prohibitin  in the MCF-7 cell lysates binds to the chromodomain and chromoshadow domain of HP1gamma while Rb binds only to the chromoshadow domain.	bind
12072	1	4779	6	NULL	NULL	NULL	NULL	Prohibitin	GP		bind					HP1gamma	GP		chromodomain		NULL	MCF-7 cell lysates	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4161_s_141	16705168	(C) Prohibitin  in the MCF-7 cell lysates binds to the chromodomain and chromoshadow domain of HP1gamma while Rb binds only to the chromoshadow domain.	bind
12073	2	4779	6	NULL	NULL	NULL	NULL	prohibitin	GP		bind					HP1gamma	GP		chromoshadow domain		NULL	MCF-7 cell lysates	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4161_s_141	16705168	(C) Prohibitin  in the MCF-7 cell lysates binds to the chromodomain and chromoshadow domain of HP1gamma while Rb binds only to the chromoshadow domain.	bind
12074	3	4779	6	NULL	NULL	NULL	NULL	Rb	GP		bind					HP1gamma	GP		chromoshadow domain		NULL	MCF-7 cell lysates	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4161_s_141	16705168	(C) Prohibitin  in the MCF-7 cell lysates binds to the chromodomain and chromoshadow domain of HP1gamma while Rb binds only to the chromoshadow domain.	bind
12075	1	4781	6	NULL	NULL	NULL	NULL	nuclear extracts	CellComponent		bind					CaSR-C	GP	radiolabeled			NULL	rMTC cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7410_s_189	9819427	(C) Protein-DNA complexes formed between nuclear extracts from rMTC cells and radiolabeled CaSR-C, CAM-III-A, CAM-III-B, E-CAD-A, or CT/CGRP-C (lanes 3 to 12) were compared to those formed with the downstream TTF-1 binding site of the TSHR (TSHR DS) (lanes 1 and 2) in the presence of an antiserum to a specific TTF-1 peptide or its preimmune control.	bind
12268	2	4781	6	NULL	NULL	NULL	NULL	nuclear extracts	CellComponent		bind					CAM-III-A	GP	radiolabeled			NULL	rMTC cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7410_s_189	9819427	(C) Protein-DNA complexes formed between nuclear extracts from rMTC cells and radiolabeled CaSR-C, CAM-III-A, CAM-III-B, E-CAD-A, or CT/CGRP-C (lanes 3 to 12) were compared to those formed with the downstream TTF-1 binding site of the TSHR (TSHR DS) (lanes 1 and 2) in the presence of an antiserum to a specific TTF-1 peptide or its preimmune control.	bind
12269	3	4781	6	NULL	NULL	NULL	NULL	nuclear extracts	CellComponent		bind					CAM-III-B	GP	radiolabeled			NULL	rMTC cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7410_s_189	9819427	(C) Protein-DNA complexes formed between nuclear extracts from rMTC cells and radiolabeled CaSR-C, CAM-III-A, CAM-III-B, E-CAD-A, or CT/CGRP-C (lanes 3 to 12) were compared to those formed with the downstream TTF-1 binding site of the TSHR (TSHR DS) (lanes 1 and 2) in the presence of an antiserum to a specific TTF-1 peptide or its preimmune control.	bind
12270	4	4781	6	NULL	NULL	NULL	NULL	nuclear extracts	CellComponent		bind					E-CAD-A	GP	radiolabeled			NULL	rMTC cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7410_s_189	9819427	(C) Protein-DNA complexes formed between nuclear extracts from rMTC cells and radiolabeled CaSR-C, CAM-III-A, CAM-III-B, E-CAD-A, or CT/CGRP-C (lanes 3 to 12) were compared to those formed with the downstream TTF-1 binding site of the TSHR (TSHR DS) (lanes 1 and 2) in the presence of an antiserum to a specific TTF-1 peptide or its preimmune control.	bind
12271	5	4781	6	NULL	NULL	NULL	NULL	nuclear extracts	CellComponent		bind					CT/CGRP-C	GP	radiolabeled			NULL	rMTC cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7410_s_189	9819427	(C) Protein-DNA complexes formed between nuclear extracts from rMTC cells and radiolabeled CaSR-C, CAM-III-A, CAM-III-B, E-CAD-A, or CT/CGRP-C (lanes 3 to 12) were compared to those formed with the downstream TTF-1 binding site of the TSHR (TSHR DS) (lanes 1 and 2) in the presence of an antiserum to a specific TTF-1 peptide or its preimmune control.	bind
12453	6	4781	6	NULL	NULL	NULL	NULL	nuclear extracts	CellComponent		bind					TSHR	GP			downstream TTF-1 binding site	NULL	rMTC cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7410_s_189	9819427	(C) Protein-DNA complexes formed between nuclear extracts from rMTC cells and radiolabeled CaSR-C, CAM-III-A, CAM-III-B, E-CAD-A, or CT/CGRP-C (lanes 3 to 12) were compared to those formed with the downstream TTF-1 binding site of the TSHR (TSHR DS) (lanes 1 and 2) in the presence of an antiserum to a specific TTF-1 peptide or its preimmune control.	bind
13939	1	4784	5	NULL	NULL	0	NULL	GFP - X-PAK5	NULL		bind	NULL				MTs	NULL				NULL	cells expressing GFP - X-PAK5 alone	0	NULL	NULL	NULL	gw60_cellbiol_155_6_1029_s_250	11733543	(C) Quantification of cells that present GFP - X-PAK5 binding to the MTs in cells expressing either GFP - X-PAK5 alone or coexpressed with active GTPases.	bind
13940	2	4784	5	NULL	NULL	0	NULL	GFP - X-PAK5	NULL		bind	NULL				MTs	NULL				NULL	in cells expressing GFP - X-PAK5 coexpressed with active GTPases	0	NULL	NULL	NULL	gw60_cellbiol_155_6_1029_s_250	11733543	(C) Quantification of cells that present GFP - X-PAK5 binding to the MTs in cells expressing either GFP - X-PAK5 alone or coexpressed with active GTPases.	bind
13941	3	4784	5	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_155_6_1029_s_250	11733543	(C) Quantification of cells that present GFP - X-PAK5 binding to the MTs in cells expressing either GFP - X-PAK5 alone or coexpressed with active GTPases.	bind
12272	1	4784	6	NULL	NULL	NULL	NULL	GFP - X-PAK5	GP		bind					MTs	CellComponent				NULL	in cells expressing GFP - X-PAK5 alone	NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_1029_s_250	11733543	(C) Quantification of cells that present GFP - X-PAK5 binding to the MTs in cells expressing either GFP - X-PAK5 alone or coexpressed with active GTPases.	bind
15193	2	4784	6	NULL	NULL	NULL	NULL	GFP - X-PAK5	GP		bind					MTs	CellComponent				NULL	in cells  expressing GFP - X-PAK5 coexpressed with active GTPases	NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_1029_s_250	11733543	(C) Quantification of cells that present GFP - X-PAK5 binding to the MTs in cells expressing either GFP - X-PAK5 alone or coexpressed with active GTPases.	bind
54506	3	4784	6	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_1029_s_250	11733543	(C) Quantification of cells that present GFP - X-PAK5 binding to the MTs in cells expressing either GFP - X-PAK5 alone or coexpressed with active GTPases.	bind
14586	1	4786	5	NULL	NULL	0	NULL	Smad4	NULL		bind	NULL					NULL			SBE/p53RE	NULL	WT mouse liver tissue	0	NULL	NULL	NULL	gw70_molcellbiol_25_3_1200_s_71	15657445	(C) Quantifying in vivo ChIP of Smad4 and P-Smad2 binding to the  SBE/p53RE and distal genomic sites in WT and p53-null mouse liver tissue.	bind
14587	2	4786	5	NULL	NULL	0	NULL	Smad4	NULL		bind	NULL					NULL			SBE/p53RE	NULL	p53-null mouse liver tissue	0	NULL	NULL	NULL	gw70_molcellbiol_25_3_1200_s_71	15657445	(C) Quantifying in vivo ChIP of Smad4 and P-Smad2 binding to the  SBE/p53RE and distal genomic sites in WT and p53-null mouse liver tissue.	bind
14588	3	4786	5	NULL	NULL	0	NULL	P-Smad2	NULL		bind	NULL					NULL			SBE/p53RE	NULL	WT mouse liver tissue	0	NULL	NULL	NULL	gw70_molcellbiol_25_3_1200_s_71	15657445	(C) Quantifying in vivo ChIP of Smad4 and P-Smad2 binding to the  SBE/p53RE and distal genomic sites in WT and p53-null mouse liver tissue.	bind
14589	4	4786	5	NULL	NULL	0	NULL	P-Smad2	NULL		bind	NULL					NULL			SBE/p53RE	NULL	p53-null mouse liver tissue	0	NULL	NULL	NULL	gw70_molcellbiol_25_3_1200_s_71	15657445	(C) Quantifying in vivo ChIP of Smad4 and P-Smad2 binding to the  SBE/p53RE and distal genomic sites in WT and p53-null mouse liver tissue.	bind
12274	1	4786	6	NULL	NULL	NULL	NULL	Smad4	GP		bind									SBE/p53RE	NULL	wild type mouse liver tissue	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_3_1200_s_71	15657445	(C) Quantifying in vivo ChIP of Smad4 and P-Smad2 binding to the  SBE/p53RE and distal genomic sites in WT and p53-null mouse liver tissue.	bind
12275	2	4786	6	NULL	NULL	NULL	NULL	Smad4	GP		bind									SBE/p53RE	NULL	p53-null mouse liver tissue	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_3_1200_s_71	15657445	(C) Quantifying in vivo ChIP of Smad4 and P-Smad2 binding to the  SBE/p53RE and distal genomic sites in WT and p53-null mouse liver tissue.	bind
12276	3	4786	6	NULL	NULL	NULL	NULL	P-Smad2	GP		bind									SBE/p53RE	NULL	wild type mouse liver tissue	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_3_1200_s_71	15657445	(C) Quantifying in vivo ChIP of Smad4 and P-Smad2 binding to the  SBE/p53RE and distal genomic sites in WT and p53-null mouse liver tissue.	bind
12277	4	4786	6	NULL	NULL	NULL	NULL	P-Smad2	GP		bind									SBE/p53RE	NULL	p53-null mouse liver tissue	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_3_1200_s_71	15657445	(C) Quantifying in vivo ChIP of Smad4 and P-Smad2 binding to the  SBE/p53RE and distal genomic sites in WT and p53-null mouse liver tissue.	bind
13942	1	4787	5	NULL	NULL	0	NULL	acetyl-histone H3	NULL		bind	NULL				bcl-2	NULL			P2 promoter	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_5_1608_s_210	15713621	(C) Quantitative ChIP  assay of acetyl-histone H3 and acetyl-histone H4 binding to the  bcl-2 P2 promoter.	bind
13943	2	4787	5	NULL	NULL	0	NULL	acetyl-histone H4	NULL		bind	NULL				bcl-2	NULL			P2 promoter	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_5_1608_s_210	15713621	(C) Quantitative ChIP  assay of acetyl-histone H3 and acetyl-histone H4 binding to the  bcl-2 P2 promoter.	bind
12310	1	4787	6	NULL	NULL	NULL	NULL	acetyl-histone H3	GP		bind					bcl-2 	GP			P2 promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1608_s_210	15713621	(C) Quantitative ChIP  assay of acetyl-histone H3 and acetyl-histone H4 binding to the  bcl-2 P2 promoter.	bind
12311	2	4787	6	NULL	NULL	NULL	NULL	acetyl-histone H4	GP		bind					bcl-2	GP			P2 promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1608_s_210	15713621	(C) Quantitative ChIP  assay of acetyl-histone H3 and acetyl-histone H4 binding to the  bcl-2 P2 promoter.	bind
13944	1	4788	5	10	NULL	0	NULL	38 kDa protein			bind					GST - BRCA1 					NULL		NULL	NULL	NULL	NULL	gw60_cell_88_2_265_s_130	9008167	(C) Rad51 antiserum recognizes a 38 kDa protein bound to  GST - BRCA1 #4.	bind
13945	2	4788	5	NULL	NULL	0	NULL	Rad51 antiserum	NULL		recognizes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_88_2_265_s_130	9008167	(C) Rad51 antiserum recognizes a 38 kDa protein bound to  GST - BRCA1 #4.	bind
12312	1	4788	6	NULL	NULL	NULL	NULL	38 kDa protein	GP		bind					GST-BRCA1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_88_2_265_s_130	9008167	(C) Rad51 antiserum recognizes a 38 kDa protein bound to  GST - BRCA1 #4.	bind
16282	2	4788	6	NULL	NULL	NULL	NULL	Rad51 antiserum	GP		recognizes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_88_2_265_s_130	9008167	(C) Rad51 antiserum recognizes a 38 kDa protein bound to  GST - BRCA1 #4.	bind
13946	1	4790	5	NULL	NULL	0	NULL	Ran-GTP	NULL		bind	NULL				Kap123p	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cell_89_5_715_s_100	9182759	(C) Ran-GTP binds to Kap123p.	bind
12313	1	4790	6	NULL	NULL	NULL	NULL	Ran-GTP	GP		bind					Kap123p	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_89_5_715_s_100	9182759	(C) Ran-GTP binds to Kap123p.	bind
14189	1	4791	5	10	NULL	0	NULL	nicotine			bind					choline acetyltransferase		activity of			NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_94_3_685_s_88	10579560	(c) Ratios of [3](-)nicotine, [3]epibatidine, [3]cytisine, and [3]vesamicol binding to choline acetyltransferase activity as averages of the individual cases.	bind
14190	2	4791	5	10	NULL	0	NULL	epibatidine			bind					choline acetyltransferase		activity of			NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_94_3_685_s_88	10579560	(c) Ratios of [3](-)nicotine, [3]epibatidine, [3]cytisine, and [3]vesamicol binding to choline acetyltransferase activity as averages of the individual cases.	bind
14191	3	4791	5	10	NULL	0	NULL	cytisine			bind					choline acetyltransferase		activity of			NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_94_3_685_s_88	10579560	(c) Ratios of [3](-)nicotine, [3]epibatidine, [3]cytisine, and [3]vesamicol binding to choline acetyltransferase activity as averages of the individual cases.	bind
14192	4	4791	5	10	NULL	0	NULL	vesamicol			bind					choline acetyltransferase		activity of			NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_94_3_685_s_88	10579560	(c) Ratios of [3](-)nicotine, [3]epibatidine, [3]cytisine, and [3]vesamicol binding to choline acetyltransferase activity as averages of the individual cases.	bind
12314	1	4791	6	NULL	NULL	NULL	NULL	nicotine	Chemical		bind					choline acetyltransferase	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_94_3_685_s_88	10579560	(c) Ratios of [3](-)nicotine, [3]epibatidine, [3]cytisine, and [3]vesamicol binding to choline acetyltransferase activity as averages of the individual cases.	bind
12315	2	4791	6	NULL	NULL	NULL	NULL	epibatidine	Chemical		bind					choline acetyltransferase	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_94_3_685_s_88	10579560	(c) Ratios of [3](-)nicotine, [3]epibatidine, [3]cytisine, and [3]vesamicol binding to choline acetyltransferase activity as averages of the individual cases.	bind
12316	3	4791	6	NULL	NULL	NULL	NULL	cytisine	AminoAcid		bind					choline acetyltransferase	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_94_3_685_s_88	10579560	(c) Ratios of [3](-)nicotine, [3]epibatidine, [3]cytisine, and [3]vesamicol binding to choline acetyltransferase activity as averages of the individual cases.	bind
12317	4	4791	6	NULL	NULL	NULL	NULL	vesamicol	Chemical		bind					choline acetyltransferase	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_94_3_685_s_88	10579560	(c) Ratios of [3](-)nicotine, [3]epibatidine, [3]cytisine, and [3]vesamicol binding to choline acetyltransferase activity as averages of the individual cases.	bind
14193	1	4792	5	NULL	NULL	0	NULL	eIF4GI	NULL	recombinant	does not bind	NULL		(1040-1560) FVR1239AAA		eIF4A	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_molcellbiol_20_2_468_s_194	10611225	(C) Recombinant eIF4GI(1040-1560) FVR1239AAA does not bind eIF4A in vitro.	bind
12318	1	4792	6	NULL	NULL	NULL	NULL	eIF4GI	GP	recombinant	does not bind			1040-1560 FVR1239AAA		eIF4A	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_2_468_s_194	10611225	(C) Recombinant eIF4GI(1040-1560) FVR1239AAA does not bind eIF4A in vitro.	bind
14194	1	4793	5	NULL	NULL	0	NULL	rhodanese	NULL	refolding of	bind	NULL				EL229C-B	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_139	11672529	(C) Refolding of rhodanese bound to EL229C-B  was initiated as in (B) followed by addition  of EL229C/SA ( ) or SR-EL/SA ( ) at 1.5 min.	bind
14196	2	4793	5	NULL	NULL	0	NULL	EL229C/SA	NULL	addition of	initiates	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_139	11672529	(C) Refolding of rhodanese bound to EL229C-B  was initiated as in (B) followed by addition  of EL229C/SA ( ) or SR-EL/SA ( ) at 1.5 min.	bind
14197	3	4793	5	NULL	NULL	0	NULL	SR-EL/SA	NULL	addition of	initiates	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_139	11672529	(C) Refolding of rhodanese bound to EL229C-B  was initiated as in (B) followed by addition  of EL229C/SA ( ) or SR-EL/SA ( ) at 1.5 min.	bind
14198	4	4793	5	NULL	NULL	0	NULL	statement 3	NULL		is an alternative to	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_139	11672529	(C) Refolding of rhodanese bound to EL229C-B  was initiated as in (B) followed by addition  of EL229C/SA ( ) or SR-EL/SA ( ) at 1.5 min.	bind
12319	1	4793	6	NULL	NULL	NULL	NULL	rhodanese	GP	refolding of	bind					EL229C-B					NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_139	11672529	(C) Refolding of rhodanese bound to EL229C-B  was initiated as in (B) followed by addition  of EL229C/SA ( ) or SR-EL/SA ( ) at 1.5 min.	bind
16283	2	4793	6	NULL	NULL	NULL	NULL	EL229C/SA		addition of	initiates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_139	11672529	(C) Refolding of rhodanese bound to EL229C-B  was initiated as in (B) followed by addition  of EL229C/SA ( ) or SR-EL/SA ( ) at 1.5 min.	bind
16284	3	4793	6	NULL	NULL	NULL	NULL	SR-EL/SA	GP	addition of	initiates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_139	11672529	(C) Refolding of rhodanese bound to EL229C-B  was initiated as in (B) followed by addition  of EL229C/SA ( ) or SR-EL/SA ( ) at 1.5 min.	bind
54507	4	4793	6	NULL	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_139	11672529	(C) Refolding of rhodanese bound to EL229C-B  was initiated as in (B) followed by addition  of EL229C/SA ( ) or SR-EL/SA ( ) at 1.5 min.	bind
14199	1	4795	5	NULL	NULL	0	NULL	[35]GTP S	NULL		bind	NULL				coronal brain sections	NULL	VEH treated mice			NULL	in caudate-putamen	0	NULL	NULL	NULL	gw70_neuropharmacology_50_7_788_s_407	16443242	(C) Representative autoradiograms for cannabinoid receptor agonist-stimulated  [35]GTP S binding of coronal brain sections from VEH and ND treated mice in the caudate-putamen.	bind
14202	2	4795	5	NULL	NULL	0	NULL	[35]GTP S	NULL		bind	NULL				coronal brain sections	NULL	ND treated mice			NULL	in caudate-putamen	0	NULL	NULL	NULL	gw70_neuropharmacology_50_7_788_s_407	16443242	(C) Representative autoradiograms for cannabinoid receptor agonist-stimulated  [35]GTP S binding of coronal brain sections from VEH and ND treated mice in the caudate-putamen.	bind
14203	3	4795	5	NULL	NULL	0	NULL	cannabinoid receptor agonist	NULL		stimulate	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_neuropharmacology_50_7_788_s_407	16443242	(C) Representative autoradiograms for cannabinoid receptor agonist-stimulated  [35]GTP S binding of coronal brain sections from VEH and ND treated mice in the caudate-putamen.	bind
14204	4	4795	5	NULL	NULL	0	NULL	cannabinoid receptor agonist	NULL		stimulate	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_neuropharmacology_50_7_788_s_407	16443242	(C) Representative autoradiograms for cannabinoid receptor agonist-stimulated  [35]GTP S binding of coronal brain sections from VEH and ND treated mice in the caudate-putamen.	bind
17054	1	4795	6	NULL	NULL	NULL	NULL	GTP S	Chemical		bind					coronal brain sections	OrganismPart	VEH treated mice 			NULL	in caudate-putamen	NULL	NULL	NULL	NULL	gw70_neuropharmacology_50_7_788_s_407	16443242	(C) Representative autoradiograms for cannabinoid receptor agonist-stimulated  [35]GTP S binding of coronal brain sections from VEH and ND treated mice in the caudate-putamen.	bind
17055	2	4795	6	NULL	NULL	NULL	NULL	GTP S	Chemical		bind					coronal brain sections	OrganismPart	ND treated mice			NULL	in caudate-putamen	NULL	NULL	NULL	NULL	gw70_neuropharmacology_50_7_788_s_407	16443242	(C) Representative autoradiograms for cannabinoid receptor agonist-stimulated  [35]GTP S binding of coronal brain sections from VEH and ND treated mice in the caudate-putamen.	bind
17057	3	4795	6	NULL	NULL	NULL	NULL	cannabinoid receptor agonist	GP		stimulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_50_7_788_s_407	16443242	(C) Representative autoradiograms for cannabinoid receptor agonist-stimulated  [35]GTP S binding of coronal brain sections from VEH and ND treated mice in the caudate-putamen.	bind
17058	4	4795	6	NULL	NULL	NULL	NULL	cannabinoid receptor agonist	GP		stimulates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_50_7_788_s_407	16443242	(C) Representative autoradiograms for cannabinoid receptor agonist-stimulated  [35]GTP S binding of coronal brain sections from VEH and ND treated mice in the caudate-putamen.	bind
14205	1	4796	5	NULL	NULL	0	NULL	ATP	NULL		bind	NULL				D2	NULL				NULL		0	NULL	NULL	NULL	gw60_genetics_155_1_203_s_121	10790395	(C) Residues involved in ATP binding by D2 are shown in contact with ATP.	bind
12320	1	4796	6	NULL	NULL	NULL	NULL	ATP	Chemical		bind					D2	GP				NULL		NULL	NULL	NULL	NULL	gw60_genetics_155_1_203_s_121	10790395	(C) Residues involved in ATP binding by D2 are shown in contact with ATP.	bind
14207	1	4797	5	NULL	NULL	0	NULL		NULL		bind	NULL		GST-RBD		RhoA	NULL				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_1_87_s_139	15527766	(C) RhoA activities are  indicated by the amount of GST-RBD bound RhoA normalized to the amount of total RhoA  content in the lysates.	bind
12321	1	4797	6	NULL	NULL	NULL	NULL				bind			GST-RBD		RhoA	GP				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_1_87_s_139	15527766	(C) RhoA activities are  indicated by the amount of GST-RBD bound RhoA normalized to the amount of total RhoA  content in the lysates.	bind
14208	1	4798	5	NULL	NULL	0	NULL	CksHs1 monomer	NULL		bind	NULL				CDK2	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_84_6_863_s_102	8601310	(C) Ribbon model of  the monomeric fold of CksHs1 monomer (yellow) bound to CDK2 (displayed as C   trace except for helix  5 and loop L14 and oriented to match   Figure 1B, with the same color code) with a superimposed CksHs2 interlocked dimer (pink  and light purple ribbons).	bind
12322	1	4798	6	NULL	NULL	NULL	NULL	CksHs1 monomer	GP		bind					CDK2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_84_6_863_s_102	8601310	(C) Ribbon model of  the monomeric fold of CksHs1 monomer (yellow) bound to CDK2 (displayed as C   trace except for helix  5 and loop L14 and oriented to match   Figure 1B, with the same color code) with a superimposed CksHs2 interlocked dimer (pink  and light purple ribbons).	bind
14209	1	4799	5	NULL	NULL	0	NULL	NF1	NULL		bind	NULL				MMTV	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_16_5417_s_168	11463824	(C) Roscovitine inhibits NF1 binding to the MMTV promoter.	bind
14210	2	4799	5	NULL	NULL	0	NULL	Roscovitine	NULL		inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_16_5417_s_168	11463824	(C) Roscovitine inhibits NF1 binding to the MMTV promoter.	bind
12323	1	4799	6	NULL	NULL	NULL	NULL	NF1	GP		bind					MMTV	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_16_5417_s_168	11463824	(C) Roscovitine inhibits NF1 binding to the MMTV promoter.	bind
12324	2	4799	6	NULL	NULL	NULL	NULL	Roscovitine	Chemical		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_16_5417_s_168	11463824	(C) Roscovitine inhibits NF1 binding to the MMTV promoter.	bind
14211	1	4801	5	NULL	NULL	0	NULL	SATB1	NULL		bind	NULL				IL2Ralpha	NULL			promoter	NULL	in vivo	0	NULL	NULL	NULL	gw70_molcellbiol_25_5_1620_s_135	15713622	(C) SATB1 binds to the IL2Ralpha promoter in vivo.	bind
12325	1	4801	6	NULL	NULL	NULL	NULL	SATB1	GP		bind					IL2Ralpha	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1620_s_135	15713622	(C) SATB1 binds to the IL2Ralpha promoter in vivo.	bind
14591	1	4802	5	10	NULL	0	NULL	Mtb HSP70		unlabeled	inhibit					FITC-Mtb HSP70		binding of			NULL		NULL	NULL	NULL	NULL	gw60_immunity_15_6_971_s_143	11754818	(C) Saturation binding of FITC-labeled Mtb HSP70 and the inhibition of FITC-Mtb HSP70 binding by unlabeled Mtb HSP70, HSA, or  E. coli HSP70.	bind
14592	2	4802	5	10	NULL	0	NULL	HSA		unlabeled	inhibit					FITC-Mtb HSP70		binding of			NULL		NULL	NULL	NULL	NULL	gw60_immunity_15_6_971_s_143	11754818	(C) Saturation binding of FITC-labeled Mtb HSP70 and the inhibition of FITC-Mtb HSP70 binding by unlabeled Mtb HSP70, HSA, or  E. coli HSP70.	bind
14593	3	4802	5	10	NULL	0	NULL	HSP70		E. coli	inhibit					FITC-Mtb HSP70		binding of			NULL		NULL	NULL	NULL	NULL	gw60_immunity_15_6_971_s_143	11754818	(C) Saturation binding of FITC-labeled Mtb HSP70 and the inhibition of FITC-Mtb HSP70 binding by unlabeled Mtb HSP70, HSA, or  E. coli HSP70.	bind
14594	4	4802	5	10	NULL	0	NULL	statement 2			is an alternative to					statement 3					NULL		NULL	NULL	NULL	NULL	gw60_immunity_15_6_971_s_143	11754818	(C) Saturation binding of FITC-labeled Mtb HSP70 and the inhibition of FITC-Mtb HSP70 binding by unlabeled Mtb HSP70, HSA, or  E. coli HSP70.	bind
12326	1	4802	6	NULL	NULL	NULL	NULL	Mtb HSP70	GP	unlabeled	inhibits					FITC-Mtb HSP70	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_immunity_15_6_971_s_143	11754818	(C) Saturation binding of FITC-labeled Mtb HSP70 and the inhibition of FITC-Mtb HSP70 binding by unlabeled Mtb HSP70, HSA, or  E. coli HSP70.	bind
12327	2	4802	6	NULL	NULL	NULL	NULL	HSA	GP	unlabeled	inhibits					FITC-Mtb HSP70	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_immunity_15_6_971_s_143	11754818	(C) Saturation binding of FITC-labeled Mtb HSP70 and the inhibition of FITC-Mtb HSP70 binding by unlabeled Mtb HSP70, HSA, or  E. coli HSP70.	bind
12328	3	4802	6	NULL	NULL	NULL	NULL	HSP70	GP	E.coli	inhibits					FITC-Mtb HSP70	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_immunity_15_6_971_s_143	11754818	(C) Saturation binding of FITC-labeled Mtb HSP70 and the inhibition of FITC-Mtb HSP70 binding by unlabeled Mtb HSP70, HSA, or  E. coli HSP70.	bind
12329	4	4802	6	NULL	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_15_6_971_s_143	11754818	(C) Saturation binding of FITC-labeled Mtb HSP70 and the inhibition of FITC-Mtb HSP70 binding by unlabeled Mtb HSP70, HSA, or  E. coli HSP70.	bind
14212	1	4803	5	10	NULL	0	NULL	NFPS			bind					GLYT1 membranes					NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_49_6_922_s_174	16143353	(C) Saturation curve of [3]NFPS binding to GLYT1 membranes.	bind
12330	1	4803	6	NULL	NULL	NULL	NULL	NFPS	Chemical		bind					GLYT1 membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_49_6_922_s_174	16143353	(C) Saturation curve of [3]NFPS binding to GLYT1 membranes.	bind
14213	1	4804	5	NULL	NULL	0	NULL	COS-7 cells	NULL		express	NULL				NP-1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cell_99_1_59_s_167	10520994	(C) Scatchard analysis of AP-Sema3A binding to NP-1- or NP-1/Plex  1 DN - expressing COS-7 cells.	bind
14214	3	4804	5	NULL	NULL	0	NULL	AP-Sema3A	NULL		bind	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cell_99_1_59_s_167	10520994	(C) Scatchard analysis of AP-Sema3A binding to NP-1- or NP-1/Plex  1 DN - expressing COS-7 cells.	bind
44572	2	4804	5	10	NULL	0	NULL	 COS-7 cells	NULL		express	NULL				NP-1/Plex 1 DN	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cell_99_1_59_s_167	10520994	(C) Scatchard analysis of AP-Sema3A binding to NP-1- or NP-1/Plex  1 DN - expressing COS-7 cells.	bind
44573	4	4804	5	10	NULL	0	NULL	AP-Sema3A	NULL		bind	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_99_1_59_s_167	10520994	(C) Scatchard analysis of AP-Sema3A binding to NP-1- or NP-1/Plex  1 DN - expressing COS-7 cells.	bind
44574	5	4804	5	10	NULL	0	NULL	statement 3	NULL		is an alternative to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_99_1_59_s_167	10520994	(C) Scatchard analysis of AP-Sema3A binding to NP-1- or NP-1/Plex  1 DN - expressing COS-7 cells.	bind
12331	1	4804	6	NULL	NULL	NULL	NULL	COS-7 cells	Cell		express					NP-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_99_1_59_s_167	10520994	(C) Scatchard analysis of AP-Sema3A binding to NP-1- or NP-1/Plex  1 DN - expressing COS-7 cells.	bind
12332	2	4804	6	NULL	NULL	NULL	NULL	COS-7 cells	Cell		express					NP-1/Plex 1 DN	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_99_1_59_s_167	10520994	(C) Scatchard analysis of AP-Sema3A binding to NP-1- or NP-1/Plex  1 DN - expressing COS-7 cells.	bind
12333	3	4804	6	NULL	NULL	NULL	NULL	AP-Sema3A	GP		bind					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_99_1_59_s_167	10520994	(C) Scatchard analysis of AP-Sema3A binding to NP-1- or NP-1/Plex  1 DN - expressing COS-7 cells.	bind
12334	5	4804	6	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_99_1_59_s_167	10520994	(C) Scatchard analysis of AP-Sema3A binding to NP-1- or NP-1/Plex  1 DN - expressing COS-7 cells.	bind
54526	4	4804	6	NULL	NULL	NULL	NULL	AP-Sema3A	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_99_1_59_s_167	10520994	(C) Scatchard analysis of AP-Sema3A binding to NP-1- or NP-1/Plex  1 DN - expressing COS-7 cells.	bind
14215	1	4805	5	NULL	NULL	0	NULL	Angiopoietin-1	NULL		bind	NULL				TIE2-Fc	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_87_7_1161_s_104	8980223	(C) Scatchard analysis of binding  of Angiopoietin-1 to TIE2-Fc.	bind
12335	1	4805	6	NULL	NULL	NULL	NULL	Angiopoietin-1	GP		bind					TIE2-Fc	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_87_7_1161_s_104	8980223	(C) Scatchard analysis of binding  of Angiopoietin-1 to TIE2-Fc.	bind
14216	1	4806	5	NULL	NULL	0	NULL	Ce-Sema1aa	NULL		bind	NULL		deltaC-Fc-AP		PLX-1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_development_129_9_2053_s_237	11959816	(C) Scatchard analysis of the binding of Ce-Sema1aadeltaC-Fc-AP to PLX-1.	bind
12336	1	4806	6	NULL	NULL	NULL	NULL	Ce-Sema1aa	GP		bind			deltaC-Fc-AP		PLX-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_development_129_9_2053_s_237	11959816	(C) Scatchard analysis of the binding of Ce-Sema1aadeltaC-Fc-AP to PLX-1.	bind
14217	1	4807	5	NULL	NULL	0	NULL	ubiquitin	NULL		bind	NULL				HAUSP	NULL		catalytic core domain		NULL		0	NULL	NULL	NULL	gw60_cell_111_7_1041_s_119	12507430	(C) Schematic diagram of how ubiquitin is bound by the HAUSP catalytic core domain.	bind
12337	1	4807	6	NULL	NULL	NULL	NULL	HAUSP	GP		bind			catalytic core domain		ubiquitin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_111_7_1041_s_119	12507430	(C) Schematic diagram of how ubiquitin is bound by the HAUSP catalytic core domain.	bind
14218	1	4812	5	10	NULL	0	NULL	 Nck			bind					PDGFR-beta		human			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_21_7867_s_197	11027258	(C) Schematic representation of binding of the two Ncks to human PDGFR-beta together with their shared binding partners.	bind
12338	1	4812	6	NULL	NULL	NULL	NULL	Nck	GP		bind					PDGFR-beta	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_21_7867_s_197	11027258	(C) Schematic representation of binding of the two Ncks to human PDGFR-beta together with their shared binding partners.	bind
14219	1	4814	5	NULL	NULL	0	NULL	agrin	NULL		bind	NULL				dystroglycan complex	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_85_4_513_s_144	8653787	(C) Schematic representation of one of several  possible models of the MuSK receptor complex for agrin, depicting requirement for a  myotube-associated specificity component (MASC) and possible interactions to additional components that may be  required for signaling or coupling to various effectors or substrates; these couplings may  be mediated extracellularly (for example, via agrin binding to the dystroglycan complex) or intracellularly  (for example, via interactions of SH2 domain - containing proteins to phosphorylated tyrosines on MuSK).	bind
14220	2	4814	5	10	NULL	0	NULL	proteins	NULL		bind	NULL		SH2 domain		MuSK	NULL	phosphorylated	tyrosines		NULL		NULL	NULL	NULL	NULL	gw60_cell_85_4_513_s_144	8653787	(C) Schematic representation of one of several  possible models of the MuSK receptor complex for agrin, depicting requirement for a  myotube-associated specificity component (MASC) and possible interactions to additional components that may be  required for signaling or coupling to various effectors or substrates; these couplings may  be mediated extracellularly (for example, via agrin binding to the dystroglycan complex) or intracellularly  (for example, via interactions of SH2 domain - containing proteins to phosphorylated tyrosines on MuSK).	bind
12339	1	4814	6	NULL	NULL	NULL	NULL	agrin	GP		bind					dystroglycan complex	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cell_85_4_513_s_144	8653787	(C) Schematic representation of one of several  possible models of the MuSK receptor complex for agrin, depicting requirement for a  myotube-associated specificity component (MASC) and possible interactions to additional components that may be  required for signaling or coupling to various effectors or substrates; these couplings may  be mediated extracellularly (for example, via agrin binding to the dystroglycan complex) or intracellularly  (for example, via interactions of SH2 domain - containing proteins to phosphorylated tyrosines on MuSK).	bind
12340	2	4814	6	NULL	NULL	NULL	NULL	protein			bind			SH2 domain		MuSK	GP	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_cell_85_4_513_s_144	8653787	(C) Schematic representation of one of several  possible models of the MuSK receptor complex for agrin, depicting requirement for a  myotube-associated specificity component (MASC) and possible interactions to additional components that may be  required for signaling or coupling to various effectors or substrates; these couplings may  be mediated extracellularly (for example, via agrin binding to the dystroglycan complex) or intracellularly  (for example, via interactions of SH2 domain - containing proteins to phosphorylated tyrosines on MuSK).	bind
14221	1	4815	5	NULL	NULL	0	NULL	Skp2	NULL		bind	NULL	selectively			p27CP	NULL				NULL	in HeLa extracts	NULL	NULL	NULL	NULL	gw60_currbiol_9_12_661_s_75	10375532	(c) Selective binding of Skp2, Skp1 and Cul-1 to p27CP in HeLa extracts.	bind
14222	2	4815	5	NULL	NULL	0	NULL	Skp1	NULL		bind	NULL	selectively			p27CP	NULL				NULL	in HeLa extracts	NULL	NULL	NULL	NULL	gw60_currbiol_9_12_661_s_75	10375532	(c) Selective binding of Skp2, Skp1 and Cul-1 to p27CP in HeLa extracts.	bind
14223	3	4815	5	NULL	NULL	0	NULL	Cul-1	NULL		bind	NULL	selectively			p27CP	NULL				NULL	in HeLa extracts	NULL	NULL	NULL	NULL	gw60_currbiol_9_12_661_s_75	10375532	(c) Selective binding of Skp2, Skp1 and Cul-1 to p27CP in HeLa extracts.	bind
12341	1	4815	6	NULL	NULL	NULL	NULL	Skp2	GP		bind		selectively			p27CP	GP				NULL	HeLa  extracts	NULL	NULL	NULL	NULL	gw60_currbiol_9_12_661_s_75	10375532	(c) Selective binding of Skp2, Skp1 and Cul-1 to p27CP in HeLa extracts.	bind
12342	2	4815	6	NULL	NULL	NULL	NULL	Skp1	GP		bind		selectively			p27CP	GP				NULL	HeLa  extracts	NULL	NULL	NULL	NULL	gw60_currbiol_9_12_661_s_75	10375532	(c) Selective binding of Skp2, Skp1 and Cul-1 to p27CP in HeLa extracts.	bind
12343	3	4815	6	NULL	NULL	NULL	NULL	Cul-1	GP		bind		selectively			p27CP	GP				NULL	HeLa  extracts	NULL	NULL	NULL	NULL	gw60_currbiol_9_12_661_s_75	10375532	(c) Selective binding of Skp2, Skp1 and Cul-1 to p27CP in HeLa extracts.	bind
14224	1	4820	5	NULL	NULL	0	NULL	NF-kappaB proteins	NULL		bind	NULL				RANTES gene	NULL			NF-kappaB binding sites within A sites	NULL		0	NULL	NULL	NULL	gw70_infectimmun_71_7_3748_s_177	12819056	(C) Sequence specificity of NF-kappaB binding activity and characterization of NF-kappaB proteins that bound to the NF-kappaB binding sites within A and B sites of the RANTES gene.	bind
14225	2	4820	5	NULL	NULL	0	NULL	NF-kappaB proteins	NULL		bind	NULL				RANTES gene	NULL			NF-kappaB binding sites within B sites	NULL		0	NULL	NULL	NULL	gw70_infectimmun_71_7_3748_s_177	12819056	(C) Sequence specificity of NF-kappaB binding activity and characterization of NF-kappaB proteins that bound to the NF-kappaB binding sites within A and B sites of the RANTES gene.	bind
12344	1	4820	6	NULL	NULL	NULL	NULL	NF-kappaB proteins	GP		bind					RANTES gene	GP			NF-kappaB binding sites within A sites	NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_71_7_3748_s_177	12819056	(C) Sequence specificity of NF-kappaB binding activity and characterization of NF-kappaB proteins that bound to the NF-kappaB binding sites within A and B sites of the RANTES gene.	bind
16285	2	4820	6	NULL	NULL	NULL	NULL	NF-kappaB proteins	GP		bind					RANTES gene	GP			NF-kappaB binding sites within B sites	NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_71_7_3748_s_177	12819056	(C) Sequence specificity of NF-kappaB binding activity and characterization of NF-kappaB proteins that bound to the NF-kappaB binding sites within A and B sites of the RANTES gene.	bind
14226	1	4821	5	NULL	NULL	0	NULL	sFRP/Frzb proteins	NULL		bind	NULL				Wnt molecules	NULL	specific			NULL		0	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
14227	2	4821	5	NULL	NULL	0	NULL	Cerberus	NULL		bind	NULL				Wnt molecules	NULL	specific			NULL		0	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
14228	3	4821	5	NULL	NULL	0	NULL	WIF-1	NULL		bind	NULL				Wnt molecules	NULL	specific			NULL		0	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
14229	4	4821	5	10	NULL	0	NULL	Wnt binding antagonists			bind					Wnt molecules		specific			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
14230	5	4821	5	NULL	NULL	0	NULL	Wnt	NULL		interacts with	NULL				Fz	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
14231	6	4821	5	NULL	NULL	0	NULL	Wnt	NULL		interacts with	NULL				LRP5/6	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
14232	7	4821	5	NULL	NULL	0	NULL	statement 5	NULL		is an alternative to	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
14235	8	4821	5	NULL	NULL	0	NULL	sFRP/Frzb proteins	NULL		prevent	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
14236	9	4821	5	NULL	NULL	0	NULL	sFRP/Frzb proteins	NULL		prevent	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
14237	10	4821	5	10	NULL	0	NULL	 sFRP/Frzb proteins			prevent					Fz-LRP5/6 complex		formation of			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
14239	11	4821	5	10	NULL	0	NULL	Cerberus			prevent					statement 5					NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
14240	12	4821	5	10	NULL	0	NULL	Cerberus			prevent					statement 6					NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
14241	13	4821	5	10	NULL	0	NULL	Cerberus			prevent					Fz-LRP5/6 complex		formation of			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
14243	16	4821	5	NULL	NULL	0	NULL	WIF-1	NULL		prevent	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
14244	17	4821	5	NULL	NULL	0	NULL	WIF-1	NULL		prevent	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
14245	18	4821	5	10	NULL	0	NULL	WIF-1			prevent					Fz-LRP5/6 complex		formation of			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
14246	19	4821	5	10	NULL	0	NULL	Wnt binding antagonists			prevent					Fz-LRP5/6 complex		formation of			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
14247	14	4821	5	10	NULL	0	NULL	Wnt binding antagonists			prevent					statement 5					NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
14248	15	4821	5	10	NULL	0	NULL	Wnt binding antagonists			prevent					statement 6					NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
12402	1	4821	6	NULL	NULL	NULL	NULL	sFRP/Frzb proteins	GP		bind					Wnt molecule	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
12403	2	4821	6	NULL	NULL	NULL	NULL	Cerberus	GP		bind					Wnt molecule	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
12404	3	4821	6	NULL	NULL	NULL	NULL	WIF-1	GP		bind					Wnt molecule	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
12436	4	4821	6	NULL	NULL	NULL	NULL	Wnt	GP		interacts with					Fz	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
12437	5	4821	6	NULL	NULL	NULL	NULL	Wnt	GP		interacts with					LRP5/6	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
12438	6	4821	6	NULL	NULL	NULL	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
12439	7	4821	6	NULL	NULL	NULL	NULL	statement 1	Process		prevents					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
12440	8	4821	6	NULL	NULL	NULL	NULL	statement 1	Process		prevents					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
12441	9	4821	6	NULL	NULL	NULL	NULL	statement 2	Process		prevents					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
12442	10	4821	6	NULL	NULL	NULL	NULL	statement 2	Process		prevents					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
12443	11	4821	6	NULL	NULL	NULL	NULL	statement 3	Process		prevents					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
12444	12	4821	6	NULL	NULL	NULL	NULL	statement 3	Process		prevents					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
12445	13	4821	6	NULL	NULL	NULL	NULL	sFRP/Frzb proteins	GP		prevents					Fz-LRP5/6 complex	GP	formation of			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
12446	14	4821	6	NULL	NULL	NULL	NULL	Cerberus	GP		prevents					Fz-LRP5/6 complex	GP	formation of			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
12447	15	4821	6	NULL	NULL	NULL	NULL	WIF-1	GP		prevents					Fz-LRP5/6 complex	GP	formation of			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
54527	16	4821	6	NULL	NULL	NULL	NULL	Wnt binding antagonists	GP		bind		specific			Wnt molecules	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
54528	17	4821	6	NULL	NULL	NULL	NULL	statement 16	Process		prevents					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
54529	18	4821	6	NULL	NULL	NULL	NULL	statement 16	Process		prevents					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
54530	19	4821	6	NULL	NULL	NULL	NULL	Wnt binding antagonists	GP		prevent					Fz-LRP5/6 complex	GP	formation of			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_275	11448771	(c) sFRP/Frzb proteins, Cerberus, WIF-1 and other Wnt binding antagonists bind specific Wnt molecules and prevent Wnt interaction with Fz and/or LRP5/6; they thereby prevent formation of the Fz-LRP5/6 complex.	bind
14251	1	4822	5	NULL	NULL	0	NULL	Ctf13	NULL		bind	NULL				Skp1	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_18_8069_s_230	15340069	(C) Sgt1 and Hsp90 stimulate the  binding of Ctf13 to Skp1.	bind
14252	2	4822	5	NULL	NULL	0	NULL	Sgt1	NULL		stimulate	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_18_8069_s_230	15340069	(C) Sgt1 and Hsp90 stimulate the  binding of Ctf13 to Skp1.	bind
14253	3	4822	5	NULL	NULL	0	NULL	Hsp90	NULL		stimulate	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_18_8069_s_230	15340069	(C) Sgt1 and Hsp90 stimulate the  binding of Ctf13 to Skp1.	bind
12405	1	4822	6	NULL	NULL	NULL	NULL	Ctf13	GP		bind					Skp1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_18_8069_s_230	15340069	(C) Sgt1 and Hsp90 stimulate the  binding of Ctf13 to Skp1.	bind
12406	2	4822	6	NULL	NULL	NULL	NULL	Sgt1	GP		stimulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_18_8069_s_230	15340069	(C) Sgt1 and Hsp90 stimulate the  binding of Ctf13 to Skp1.	bind
12407	3	4822	6	NULL	NULL	NULL	NULL	Hsp90	GP		stimulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_18_8069_s_230	15340069	(C) Sgt1 and Hsp90 stimulate the  binding of Ctf13 to Skp1.	bind
14254	1	4825	5	NULL	NULL	0	NULL	MazE	NULL		bind	NULL		random coil region between strand S4 and helix H2		MazF	NULL		helix H3		NULL		0	NULL	NULL	NULL	gw60_molcell_11_4_875_s_157	12718874	(C) Site 3: the random coil region of MazE between   strand S4 and   helix H2 bound to   helix H3 of MazF.	bind
12408	1	4825	6	NULL	NULL	NULL	NULL	MazE	GP		bind			random coil region between strand S4 and helix H2		MazF	GP		helix H3		NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_4_875_s_157	12718874	(C) Site 3: the random coil region of MazE between   strand S4 and   helix H2 bound to   helix H3 of MazF.	bind
14257	2	4827	5	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL				Ctpct probe	NULL			single binding elements	NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_41_4_583_s_125	10744779	(C) Sp proteins transiently expressed in SL2 cells bind to the  Ctpct probe containing single binding elements.	bind
44575	1	4827	5	10	NULL	0	NULL	SL2 cells	NULL		express	NULL	transiently			Sp proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_41_4_583_s_125	10744779	(C) Sp proteins transiently expressed in SL2 cells bind to the  Ctpct probe containing single binding elements.	bind
12409	1	4827	6	NULL	NULL	NULL	NULL	SL2 cells	Cell		express		transiently			Sp proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_41_4_583_s_125	10744779	(C) Sp proteins transiently expressed in SL2 cells bind to the  Ctpct probe containing single binding elements.	bind
12410	2	4827	6	NULL	NULL	NULL	NULL	statement 1	Process		bind					Ctpct probe	NucleicAcid			single binding elements	NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_41_4_583_s_125	10744779	(C) Sp proteins transiently expressed in SL2 cells bind to the  Ctpct probe containing single binding elements.	bind
14258	1	4829	5	NULL	NULL	0	NULL	NF-kappaB	NULL		bind	NULL	specifically			cyclin D1	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_4_2690_s_106	10082535	(C) Specific binding of NF-kappaB to the cyclin D1 promoter.	bind
12411	1	4829	6	NULL	NULL	NULL	NULL	NF-kappaB	GP		bind		specifically			cyclin D1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_2690_s_106	10082535	(C) Specific binding of NF-kappaB to the cyclin D1 promoter.	bind
14259	1	4830	5	NULL	NULL	0	NULL	SE RNA #1	NULL		bind	NULL	specifically			NFATc	NULL		DBD		NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_298_4_486_s_69	12408978	(C) Specific binding of SE RNA #1 to NFATc DBD.	bind
12412	1	4830	6	NULL	NULL	NULL	NULL	SE RNA #1	NucleicAcid		bind		specifically			NFATc	GP		DBD		NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_298_4_486_s_69	12408978	(C) Specific binding of SE RNA #1 to NFATc DBD.	bind
14260	1	4831	5	NULL	NULL	0	NULL	LXR	NULL		bind	NULL	specifically		PPRE	PPAR /RXR heterodimers	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_1_161_s_69	11172721	(C) Specific binding of the LXR  PPRE by PPAR /RXR heterodimers.	bind
12413	1	4831	6	NULL	NULL	NULL	NULL	PPAR /RXR heterodimers	GP		bind		specifically			LXR	GP			PPRE	NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_1_161_s_69	11172721	(C) Specific binding of the LXR  PPRE by PPAR /RXR heterodimers.	bind
14261	1	4832	5	NULL	NULL	0	NULL	TAR RNA	NULL		bind	NULL				NC protein	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_4_1181_s_92	15249214	(C) Specific inhibition by aptamer N70-13 of TAR  RNA binding to NC protein.	bind
14262	2	4832	5	NULL	NULL	0	NULL	aptamer N70-13	NULL		inhibit	NULL	specifically			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_4_1181_s_92	15249214	(C) Specific inhibition by aptamer N70-13 of TAR  RNA binding to NC protein.	bind
12414	1	4832	6	NULL	NULL	NULL	NULL	TAR RNA	NucleicAcid		bind					NC protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_4_1181_s_92	15249214	(C) Specific inhibition by aptamer N70-13 of TAR  RNA binding to NC protein.	bind
12415	2	4832	6	NULL	NULL	NULL	NULL	aptamer N70-13	NucleicAcid		inhibit		specifically			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_4_1181_s_92	15249214	(C) Specific inhibition by aptamer N70-13 of TAR  RNA binding to NC protein.	bind
14263	1	4833	5	NULL	NULL	0	NULL	XAP1	NULL		bind	NULL				CRM1	NULL				NULL		0	NULL	NULL	NULL	gw60_chembiol_7_5_345_s_62	10801471	(c) Specificity of XAP1 binding to CRM1.	bind
12416	1	4833	6	NULL	NULL	NULL	NULL	XAP1	GP		bind					CRM1	GP				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_7_5_345_s_62	10801471	(c) Specificity of XAP1 binding to CRM1.	bind
14264	1	4836	5	NULL	NULL	0	NULL	Stat5a dimers	NULL		bind	NULL				M10 PRRIII probe	NULL	mutant			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_3_1910_s_165	10022878	(C) Stat5a and Stat5b can bind to the mutant M10 PRRIII probe equally well as dimers and 2x dimers.	bind
14265	2	4836	5	NULL	NULL	0	NULL	Stat5a 2x dimers	NULL		bind	NULL				M10 PRRIII probe	NULL	mutant			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_3_1910_s_165	10022878	(C) Stat5a and Stat5b can bind to the mutant M10 PRRIII probe equally well as dimers and 2x dimers.	bind
14266	3	4836	5	NULL	NULL	0	NULL	Stat5b dimers	NULL		bind	NULL				M10 PRRIII probe	NULL	mutant			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_1910_s_165	10022878	(C) Stat5a and Stat5b can bind to the mutant M10 PRRIII probe equally well as dimers and 2x dimers.	bind
14267	4	4836	5	NULL	NULL	0	NULL	Stat5b 2x dimers	NULL		bind	NULL				M10 PRRIII probe	NULL	mutant			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_1910_s_165	10022878	(C) Stat5a and Stat5b can bind to the mutant M10 PRRIII probe equally well as dimers and 2x dimers.	bind
54536	5	4836	5	10	NULL	0	NULL	statement 1		binding of	is equivalent to					statement 2		binding of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_3_1910_s_165	10022878	(C) Stat5a and Stat5b can bind to the mutant M10 PRRIII probe equally well as dimers and 2x dimers.	bind
54537	6	4836	5	10	NULL	0	NULL	statement 3		binding of	is equivalent to					statement 4		binding of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_3_1910_s_165	10022878	(C) Stat5a and Stat5b can bind to the mutant M10 PRRIII probe equally well as dimers and 2x dimers.	bind
12417	1	4836	6	NULL	NULL	NULL	NULL	Stat5a dimers	GP		bind					M10 PRRIII probe	NucleicAcid	mutant			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_1910_s_165	10022878	(C) Stat5a and Stat5b can bind to the mutant M10 PRRIII probe equally well as dimers and 2x dimers.	bind
12418	2	4836	6	NULL	NULL	NULL	NULL	Stat5b dimers	GP		bind					M10 PRRIII probe	NucleicAcid	mutant			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_1910_s_165	10022878	(C) Stat5a and Stat5b can bind to the mutant M10 PRRIII probe equally well as dimers and 2x dimers.	bind
54534	3	4836	6	NULL	NULL	NULL	NULL	Stat5a 2x dimers	GP		bind					M10 PRRIII probe	NucleicAcid	mutant			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_1910_s_165	10022878	(C) Stat5a and Stat5b can bind to the mutant M10 PRRIII probe equally well as dimers and 2x dimers.	bind
54535	4	4836	6	NULL	NULL	NULL	NULL	Stat5b 2xdimers	GP		bind					M10 PRRIII probe	NucleicAcid	mutant			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_1910_s_165	10022878	(C) Stat5a and Stat5b can bind to the mutant M10 PRRIII probe equally well as dimers and 2x dimers.	bind
54538	5	4836	6	NULL	NULL	NULL	NULL	statement 1	Process	binding of	is equivalent to					statement 3	Process	binding of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_1910_s_165	10022878	(C) Stat5a and Stat5b can bind to the mutant M10 PRRIII probe equally well as dimers and 2x dimers.	bind
54539	6	4836	6	NULL	NULL	NULL	NULL	statement 2	Process	binding of	is equivalent to					statement 4	Process	binding of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_1910_s_165	10022878	(C) Stat5a and Stat5b can bind to the mutant M10 PRRIII probe equally well as dimers and 2x dimers.	bind
14268	1	4837	5	NULL	NULL	0	NULL	GTP S	NULL		bind	NULL				myr-bARF1	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_molcell_3_3_275_s_73	10198630	(C) Strains listed in (B) were incubated with or without BFA (100  g/mL) for 2 min, pulse labeled for 10 min, and chased for 30 min. (D) Inhibition of Gea1p or G-AR-Gp chimera-stimulated GTP S binding to myr-bARF1 by BFA in vitro was monitored.	bind
14269	2	4837	5	NULL	NULL	0	NULL	Gea1p	NULL		stimulate	NULL				statement 1	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_molcell_3_3_275_s_73	10198630	(C) Strains listed in (B) were incubated with or without BFA (100  g/mL) for 2 min, pulse labeled for 10 min, and chased for 30 min. (D) Inhibition of Gea1p or G-AR-Gp chimera-stimulated GTP S binding to myr-bARF1 by BFA in vitro was monitored.	bind
14270	3	4837	5	NULL	NULL	0	NULL	G-AR-Gp chimera	NULL		stimulate	NULL				statement 1	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_molcell_3_3_275_s_73	10198630	(C) Strains listed in (B) were incubated with or without BFA (100  g/mL) for 2 min, pulse labeled for 10 min, and chased for 30 min. (D) Inhibition of Gea1p or G-AR-Gp chimera-stimulated GTP S binding to myr-bARF1 by BFA in vitro was monitored.	bind
14271	4	4837	5	NULL	NULL	0	NULL	BFA	NULL		inhibit	NULL				statement 2	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_molcell_3_3_275_s_73	10198630	(C) Strains listed in (B) were incubated with or without BFA (100  g/mL) for 2 min, pulse labeled for 10 min, and chased for 30 min. (D) Inhibition of Gea1p or G-AR-Gp chimera-stimulated GTP S binding to myr-bARF1 by BFA in vitro was monitored.	bind
14272	5	4837	5	NULL	NULL	0	NULL	BFA	NULL		inhibit	NULL				statement 3	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_molcell_3_3_275_s_73	10198630	(C) Strains listed in (B) were incubated with or without BFA (100  g/mL) for 2 min, pulse labeled for 10 min, and chased for 30 min. (D) Inhibition of Gea1p or G-AR-Gp chimera-stimulated GTP S binding to myr-bARF1 by BFA in vitro was monitored.	bind
12419	1	4837	6	NULL	NULL	NULL	NULL	GTP S 	GP		bind					myr-bARF1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcell_3_3_275_s_73	10198630	(C) Strains listed in (B) were incubated with or without BFA (100  g/mL) for 2 min, pulse labeled for 10 min, and chased for 30 min. (D) Inhibition of Gea1p or G-AR-Gp chimera-stimulated GTP S binding to myr-bARF1 by BFA in vitro was monitored.	bind
54545	2	4837	6	NULL	NULL	NULL	NULL	Gea1p	GP		stimulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_3_275_s_73	10198630	(C) Strains listed in (B) were incubated with or without BFA (100  g/mL) for 2 min, pulse labeled for 10 min, and chased for 30 min. (D) Inhibition of Gea1p or G-AR-Gp chimera-stimulated GTP S binding to myr-bARF1 by BFA in vitro was monitored.	bind
54546	3	4837	6	NULL	NULL	NULL	NULL	G-AR-Gp chimera	GP		stimulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_3_275_s_73	10198630	(C) Strains listed in (B) were incubated with or without BFA (100  g/mL) for 2 min, pulse labeled for 10 min, and chased for 30 min. (D) Inhibition of Gea1p or G-AR-Gp chimera-stimulated GTP S binding to myr-bARF1 by BFA in vitro was monitored.	bind
54547	4	4837	6	NULL	NULL	NULL	NULL	BFA	GP		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_3_275_s_73	10198630	(C) Strains listed in (B) were incubated with or without BFA (100  g/mL) for 2 min, pulse labeled for 10 min, and chased for 30 min. (D) Inhibition of Gea1p or G-AR-Gp chimera-stimulated GTP S binding to myr-bARF1 by BFA in vitro was monitored.	bind
54548	5	4837	6	NULL	NULL	NULL	NULL	BFA	GP		inhibit					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_3_275_s_73	10198630	(C) Strains listed in (B) were incubated with or without BFA (100  g/mL) for 2 min, pulse labeled for 10 min, and chased for 30 min. (D) Inhibition of Gea1p or G-AR-Gp chimera-stimulated GTP S binding to myr-bARF1 by BFA in vitro was monitored.	bind
14273	1	4839	5	10	NULL	0	NULL	ARF	NULL		bind	NULL				N5 fragment	NULL	wild-type		nodal ASE	NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_1_35_s_193	10678167	(C) Supershift analysis of ARF binding to the  N5  wild-type fragment of  nodal ASE.	bind
12420	1	4839	6	NULL	NULL	NULL	NULL	ARF	GP		bind					 N5 fragment	NucleicAcid	wild-type		nodal ASE	NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_1_35_s_193	10678167	(C) Supershift analysis of ARF binding to the  N5  wild-type fragment of  nodal ASE.	bind
14274	1	4840	5	NULL	NULL	0	NULL	HNF1	NULL		bind	NULL					NULL			HNF1 element	NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_311_1_233_s_92	14575719	(C) Supershift experiments carried out with  antibodies to HNF1  and HNF1  indicate that HNF1  is binding to the HNF1 element.	bind
12421	1	4840	6	NULL	NULL	NULL	NULL	HNF1	GP		bind									HNF1 element	NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_311_1_233_s_92	14575719	(C) Supershift experiments carried out with  antibodies to HNF1  and HNF1  indicate that HNF1  is binding to the HNF1 element.	bind
14275	1	4841	5	NULL	NULL	0	NULL	Taf1p	NULL		bind	NULL				HXT	NULL				NULL	in Wt cells	0	NULL	NULL	NULL	gw70_molcellbiol_25_12_4863_s_174	15923605	(C) Taf1p binding to  HXT in Wt,  gcn5delta,  spt3delta, and  spt8delta cells.	bind
14276	2	4841	5	NULL	NULL	0	NULL	Taf1p	NULL		bind	NULL				HXT 	NULL				NULL	in gcn5delta cells	0	NULL	NULL	NULL	gw70_molcellbiol_25_12_4863_s_174	15923605	(C) Taf1p binding to  HXT in Wt,  gcn5delta,  spt3delta, and  spt8delta cells.	bind
14277	3	4841	5	NULL	NULL	0	NULL	Taf1p	NULL		bind	NULL				HXT	NULL				NULL	in spt3delta cells	0	NULL	NULL	NULL	gw70_molcellbiol_25_12_4863_s_174	15923605	(C) Taf1p binding to  HXT in Wt,  gcn5delta,  spt3delta, and  spt8delta cells.	bind
14278	4	4841	5	NULL	NULL	0	NULL	Taf1p	NULL		bind	NULL				HXT	NULL				NULL	in spt8delta cells	0	NULL	NULL	NULL	gw70_molcellbiol_25_12_4863_s_174	15923605	(C) Taf1p binding to  HXT in Wt,  gcn5delta,  spt3delta, and  spt8delta cells.	bind
12422	1	4841	6	NULL	NULL	NULL	NULL	Taf1p	GP		bind					HXT	GP				NULL	wild type cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_4863_s_174	15923605	(C) Taf1p binding to  HXT in Wt,  gcn5delta,  spt3delta, and  spt8delta cells.	bind
12423	2	4841	6	NULL	NULL	NULL	NULL	Taf1p	GP		bind					HXT	GP				NULL	gcn5delta cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_4863_s_174	15923605	(C) Taf1p binding to  HXT in Wt,  gcn5delta,  spt3delta, and  spt8delta cells.	bind
12424	3	4841	6	NULL	NULL	NULL	NULL	Taf1p	GP		bind					HXT	GP				NULL	spt3delta cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_4863_s_174	15923605	(C) Taf1p binding to  HXT in Wt,  gcn5delta,  spt3delta, and  spt8delta cells.	bind
12425	4	4841	6	NULL	NULL	NULL	NULL	Taf1p	GP		bind					HXT	GP				NULL	spt8delta cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_4863_s_174	15923605	(C) Taf1p binding to  HXT in Wt,  gcn5delta,  spt3delta, and  spt8delta cells.	bind
14279	1	4842	5	NULL	NULL	0	NULL	TAL1beta-BM	NULL		does not bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_12_6939_s_298	9819382	(C) TAL1beta-BM does not bind to DNA. 293E cells were transfected with expression vectors for wild-type or mutant TAL1beta and E47S.	bind
12426	1	4842	6	NULL	NULL	NULL	NULL	TAL1beta-BM	GP		does not bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6939_s_298	9819382	(C) TAL1beta-BM does not bind to DNA. 293E cells were transfected with expression vectors for wild-type or mutant TAL1beta and E47S.	bind
14280	1	4843	5	NULL	NULL	0	NULL	oligomer mut 4	NULL		contains	NULL				mutated 3' end of the binding motif	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_8_5823_s_283	10409768	(C) TASS-1 binds weakly to oligomers mut 4 and mut 5, in which the 3' end of the binding motif has been mutated (solid box); however, Co-F cannot bind to the DNA-TASS-1 complex.	bind
14281	2	4843	5	NULL	NULL	0	NULL	oligomer mut 5	NULL		contains	NULL				mutated 3' end of the binding motif	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_8_5823_s_283	10409768	(C) TASS-1 binds weakly to oligomers mut 4 and mut 5, in which the 3' end of the binding motif has been mutated (solid box); however, Co-F cannot bind to the DNA-TASS-1 complex.	bind
14282	3	4843	5	NULL	NULL	0	NULL	TASS-1	NULL		bind	NULL	weakly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_8_5823_s_283	10409768	(C) TASS-1 binds weakly to oligomers mut 4 and mut 5, in which the 3' end of the binding motif has been mutated (solid box); however, Co-F cannot bind to the DNA-TASS-1 complex.	bind
14283	4	4843	5	NULL	NULL	0	NULL	TASS-1	NULL		bind	NULL	weakly			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_8_5823_s_283	10409768	(C) TASS-1 binds weakly to oligomers mut 4 and mut 5, in which the 3' end of the binding motif has been mutated (solid box); however, Co-F cannot bind to the DNA-TASS-1 complex.	bind
14284	5	4843	5	NULL	NULL	0	NULL	Co-F	NULL		does not bind	NULL				DNA-TASS-1 complex	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_8_5823_s_283	10409768	(C) TASS-1 binds weakly to oligomers mut 4 and mut 5, in which the 3' end of the binding motif has been mutated (solid box); however, Co-F cannot bind to the DNA-TASS-1 complex.	bind
12427	1	4843	6	NULL	NULL	NULL	NULL	TASS-1	GP		bind		weakly			mut 4 oligomer	NucleicAcid	mutant	3' end of the binding motif		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5823_s_283	10409768	(C) TASS-1 binds weakly to oligomers mut 4 and mut 5, in which the 3' end of the binding motif has been mutated (solid box); however, Co-F cannot bind to the DNA-TASS-1 complex.	bind
12428	2	4843	6	NULL	NULL	NULL	NULL	TASS-1	GP		bind		weakly			mut 5 oligomer	NucleicAcid	mutant	3' end of the binding motif		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5823_s_283	10409768	(C) TASS-1 binds weakly to oligomers mut 4 and mut 5, in which the 3' end of the binding motif has been mutated (solid box); however, Co-F cannot bind to the DNA-TASS-1 complex.	bind
12429	3	4843	6	NULL	NULL	NULL	NULL	Co-F	GP		does not bind					DNA-TASS-1 complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5823_s_283	10409768	(C) TASS-1 binds weakly to oligomers mut 4 and mut 5, in which the 3' end of the binding motif has been mutated (solid box); however, Co-F cannot bind to the DNA-TASS-1 complex.	bind
14285	1	4844	5	NULL	NULL	0	NULL	TCR-CD3	NULL		bind	NULL				Nck	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_109_7_901_s_136	12110186	(C) TCR-CD3 binding to Nck is detected before protein tyrosine phosphorylation.	bind
14286	2	4844	5	NULL	NULL	0	NULL	statement 1	NULL		occurs before	NULL				protein	NULL	phosphorylation of	tyrosine		NULL		0	NULL	NULL	NULL	gw60_cell_109_7_901_s_136	12110186	(C) TCR-CD3 binding to Nck is detected before protein tyrosine phosphorylation.	bind
12430	1	4844	6	NULL	NULL	NULL	NULL	TCR-CD3	GP		bind					Nck	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_109_7_901_s_136	12110186	(C) TCR-CD3 binding to Nck is detected before protein tyrosine phosphorylation.	bind
16286	2	4844	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs before					 protein	GP	phosphorylation of	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_cell_109_7_901_s_136	12110186	(C) TCR-CD3 binding to Nck is detected before protein tyrosine phosphorylation.	bind
14287	1	4845	5	NULL	NULL	0	NULL	TCR	NULL		bind	NULL				peptide-MHC complexes	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_5_10_1116_s_56	8548281	(c) The    TCR binds peptide-MHC complexes.	bind
12431	1	4845	6	NULL	NULL	NULL	NULL	TCR	GP		bind					peptide-MHC complexes	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_5_10_1116_s_56	8548281	(c) The    TCR binds peptide-MHC complexes.	bind
54549	1	4846	5	10	NULL	0	NULL	annexin V			bind					PI					NULL		0	NULL	NULL	NULL	gw70_cellbiol_173_1_133_s_61	16606695	(C) The  duration from rounding to annexin V binding and annexin V binding to PI uptake was  calculated for individual cells and is presented as means  plus-or-minus  SEM (error  bars;  n = 25).	bind
12432	1	4846	6	NULL	NULL	NULL	NULL	annexin V	GP		bind					PI	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_1_133_s_61	16606695	(C) The  duration from rounding to annexin V binding and annexin V binding to PI uptake was  calculated for individual cells and is presented as means  plus-or-minus  SEM (error  bars;  n = 25).	bind
14288	1	4847	5	NULL	NULL	0	NULL	p27	NULL	cellular	bind	NULL				CRM1	NULL	recombinant			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_1_201_s_192	12529437	(C) The  effect of LMB on binding of recombinant CRM1 to cellular p27 was assayed as in A.  Equal amounts of heat stable p27 recovered from midG1 cells were reacted with recombinant  RanGTP and CRM1 without (lane 1) or with (lane 2) pretreatment of the CRM1 with LMB.	bind
12433	1	4847	6	NULL	NULL	NULL	NULL	CRM1	GP	recombinant	bind					p27	GP	cellular			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_1_201_s_192	12529437	(C) The  effect of LMB on binding of recombinant CRM1 to cellular p27 was assayed as in A.  Equal amounts of heat stable p27 recovered from midG1 cells were reacted with recombinant  RanGTP and CRM1 without (lane 1) or with (lane 2) pretreatment of the CRM1 with LMB.	bind
14289	1	4848	5	NULL	NULL	0	NULL	Daxx	NULL		bind	NULL		acidic domain		p53	NULL		COOH terminus		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_1_322_s_122	12482984	(C) The acidic domain of Daxx binds to the COOH terminus of p53.	bind
12434	1	4848	6	NULL	NULL	NULL	NULL	Daxx	GP		bind			acidic domain		p53	GP		COOH terminus		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_1_322_s_122	12482984	(C) The acidic domain of Daxx binds to the COOH terminus of p53.	bind
14290	1	4849	5	NULL	NULL	0	NULL	axin	NULL		bind	NULL		GID		GSK-3beta	NULL				NULL	in oocytes	0	NULL	NULL	NULL	gw60_molcellbiol_19_10_7147_s_100	10490650	(C) The axin GID binds GSK-3beta in oocytes.	bind
12435	1	4849	6	NULL	NULL	NULL	NULL	axin	GP		bind			GID		GSK-3beta	GP				NULL	oocytes	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_7147_s_100	10490650	(C) The axin GID binds GSK-3beta in oocytes.	bind
16291	1	4850	5	10	NULL	0	NULL			bidirectional	require				BAL1/BBAP promoter 			intact		IRF-1 binding site	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_14_5348_s_214	16809771	(C) The bidirectional  BAL1/BBAP promoter requires intact IRF-1 and STAT binding sites for IFN-gamma-induced activity.	bind
16292	2	4850	5	10	NULL	0	NULL			bidirectional	require				BAL1/BBAP promoter	IFN-gamma		induced activity of		STAT binding sites	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_14_5348_s_214	16809771	(C) The bidirectional  BAL1/BBAP promoter requires intact IRF-1 and STAT binding sites for IFN-gamma-induced activity.	bind
41611	1	4850	6	NULL	NULL	NULL	NULL			bidirectional	requires				BAL1/BBAP promoter					IRF-1 binding site	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_14_5348_s_214	16809771	(C) The bidirectional  BAL1/BBAP promoter requires intact IRF-1 and STAT binding sites for IFN-gamma-induced activity.	bind
41612	2	4850	6	NULL	NULL	NULL	NULL			bidirectional	 require				BAL1/BBAP promoter	IFN-gamma	GP	induced activity of		STAT binding sites	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_14_5348_s_214	16809771	(C) The bidirectional  BAL1/BBAP promoter requires intact IRF-1 and STAT binding sites for IFN-gamma-induced activity.	bind
14291	1	4851	5	NULL	NULL	0	NULL	ATRIP-LG	NULL		bind	NULL				ATR	NULL				NULL	in A549-derived cells	0	NULL	NULL	NULL	gw70_molbiolcell_16_12_5551_s_88	16176973	(C) The binding ability of ATRIP-LG to ATR. A549-derived cells were lysed  and subjected to immunoprecipitation using anti-ATR or anti-Myc antibody.	bind
12454	1	4851	6	NULL	NULL	NULL	NULL	ATRIP-LG	GP		bind					ATR	GP				NULL	A549-derived cells	NULL	NULL	NULL	NULL	gw70_molbiolcell_16_12_5551_s_88	16176973	(C) The binding ability of ATRIP-LG to ATR. A549-derived cells were lysed  and subjected to immunoprecipitation using anti-ATR or anti-Myc antibody.	bind
14294	1	4853	5	NULL	NULL	0	NULL	p53	NULL		bind	NULL				Ankyrin-like repeat protein gene	NULL			promoter	NULL	primary MEF	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_9_3492_s_219	16611991	(C) The binding of p53 to the  Ankyrin-like repeat protein gene promoter was compared in primary and transformed MEFs.	bind
44588	2	4853	5	10	NULL	0	NULL	p53	NULL		bind	NULL				Ankyrin-like repeat protein gene	NULL			promoter	NULL	transformed MEFs	0	NULL	NULL	NULL	gw70_molcellbiol_26_9_3492_s_219	16611991	(C) The binding of p53 to the  Ankyrin-like repeat protein gene promoter was compared in primary and transformed MEFs.	bind
12455	1	4853	6	NULL	NULL	NULL	NULL	p53	GP		bind					Ankyrin-like repeat protein gene	GP			promoter	NULL	primary MEF	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_9_3492_s_219	16611991	(C) The binding of p53 to the  Ankyrin-like repeat protein gene promoter was compared in primary and transformed MEFs.	bind
12456	2	4853	6	NULL	NULL	NULL	NULL	p53	GP		bind					Ankyrin-like repeat protein gene	GP			promoter	NULL	transformed MEF	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_9_3492_s_219	16611991	(C) The binding of p53 to the  Ankyrin-like repeat protein gene promoter was compared in primary and transformed MEFs.	bind
14295	1	4854	5	NULL	NULL	0	NULL	DHM5	NULL		is	NULL				truncated myosin-Va	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_194	16030255	(C) The binding of truncated myosin-Va  (DHM5) by syntaxin-1A requires a pCa of 6.6.	bind
14296	2	4854	5	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL				syntaxin-1A	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_194	16030255	(C) The binding of truncated myosin-Va  (DHM5) by syntaxin-1A requires a pCa of 6.6.	bind
12457	1	4854	6	NULL	NULL	NULL	NULL	myosin-Va	GP	truncated	bind					syntaxin-1A	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_194	16030255	(C) The binding of truncated myosin-Va  (DHM5) by syntaxin-1A requires a pCa of 6.6.	bind
16299	2	4854	6	NULL	NULL	NULL	NULL	myosin-Va	GP	truncated	is					DHM5	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_194	16030255	(C) The binding of truncated myosin-Va  (DHM5) by syntaxin-1A requires a pCa of 6.6.	bind
14298	1	4855	5	NULL	NULL	0	NULL	p97	NULL	wt	bind	NULL				p62	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_8_12_2379_s_213	9398662	(C) The binding of wt p97 and deltaN p97 to p62 adsorbed to microtiter wells was analyzed as in panel B.	bind
14299	2	4855	5	NULL	NULL	0	NULL	p97	NULL		bind	NULL		deltaN		p62	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_8_12_2379_s_213	9398662	(C) The binding of wt p97 and deltaN p97 to p62 adsorbed to microtiter wells was analyzed as in panel B.	bind
12589	1	4855	6	NULL	NULL	NULL	NULL	p97	GP	wild type	bind					p62	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_8_12_2379_s_213	9398662	(C) The binding of wt p97 and deltaN p97 to p62 adsorbed to microtiter wells was analyzed as in panel B.	bind
12590	2	4855	6	NULL	NULL	NULL	NULL	p97	GP		bind			deltaN		p62	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_8_12_2379_s_213	9398662	(C) The binding of wt p97 and deltaN p97 to p62 adsorbed to microtiter wells was analyzed as in panel B.	bind
14300	1	4856	5	NULL	NULL	0	NULL	NBS1	NULL	Xenopus	bind	NULL		C-terminal 50 amino acid		ATM	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_13_5363_s_234	15964794	(C) The C-terminal 50 amino acids  of  Xenopus NBS1 bind ATM but not Mre11, whereas the C-terminal 147 amino acids of NBS1 bind  to both ATM and Mre11.	bind
14301	2	4856	5	NULL	NULL	0	NULL	NBS1	NULL	Xenopus	does not bind	NULL		C-terminal 50 amino acids		Mre11	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_13_5363_s_234	15964794	(C) The C-terminal 50 amino acids  of  Xenopus NBS1 bind ATM but not Mre11, whereas the C-terminal 147 amino acids of NBS1 bind  to both ATM and Mre11.	bind
14302	3	4856	5	10	NULL	0	NULL	NBS1		Xenopus	bind			C-terminal 147 amino acids		ATM					NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5363_s_234	15964794	(C) The C-terminal 50 amino acids  of  Xenopus NBS1 bind ATM but not Mre11, whereas the C-terminal 147 amino acids of NBS1 bind  to both ATM and Mre11.	bind
14303	4	4856	5	10	NULL	0	NULL	NBS1		Xenopus	bind			C-terminal 147 amino acids		Mre11					NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5363_s_234	15964794	(C) The C-terminal 50 amino acids  of  Xenopus NBS1 bind ATM but not Mre11, whereas the C-terminal 147 amino acids of NBS1 bind  to both ATM and Mre11.	bind
12591	1	4856	6	NULL	NULL	NULL	NULL	NBS1	GP	Xenopus	bind			C-terminal 50 amino acids 		ATM	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5363_s_234	15964794	(C) The C-terminal 50 amino acids  of  Xenopus NBS1 bind ATM but not Mre11, whereas the C-terminal 147 amino acids of NBS1 bind  to both ATM and Mre11.	bind
12592	2	4856	6	NULL	NULL	NULL	NULL	NBS1	GP	Xenopus	does not bind			C-terminal 50 amino acids		Mre11	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5363_s_234	15964794	(C) The C-terminal 50 amino acids  of  Xenopus NBS1 bind ATM but not Mre11, whereas the C-terminal 147 amino acids of NBS1 bind  to both ATM and Mre11.	bind
12593	3	4856	6	NULL	NULL	NULL	NULL	NBS1	GP	Xenopus	bind			C-terminal 147 amino acids		ATM	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5363_s_234	15964794	(C) The C-terminal 50 amino acids  of  Xenopus NBS1 bind ATM but not Mre11, whereas the C-terminal 147 amino acids of NBS1 bind  to both ATM and Mre11.	bind
12594	4	4856	6	NULL	NULL	NULL	NULL	NBS1	GP	Xenopus	bind			C-terminal 147 amino acids		Mre11	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5363_s_234	15964794	(C) The C-terminal 50 amino acids  of  Xenopus NBS1 bind ATM but not Mre11, whereas the C-terminal 147 amino acids of NBS1 bind  to both ATM and Mre11.	bind
14304	1	4857	5	10	NULL	0	NULL	CheY			bind					CheA			P2 domain		NULL		NULL	NULL	NULL	NULL	gw60_molcell_2_4_485_s_155	9809070	(c) The CheY binding P2 domain of CheA has an  /  structure.	bind
14305	1	4858	5	10	NULL	0	NULL	Vav S3			is					Vav protein  		mutant;;lacking	C-terminal SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_6_729_s_58	10394361	(C) The CN from HIV fails to bind to the mutant Vav protein lacking the C-terminal SH3 domain (Vav S3) (lanes 5-8) but interacts with Vav2 (lanes 1-4) in COS cells.	bind
14306	2	4858	5	NULL	NULL	0	NULL	CN	NULL	 HIV	does not bind	NULL				Vav S3	NULL				NULL	in COS cells	NULL	NULL	NULL	NULL	gw60_molcell_3_6_729_s_58	10394361	(C) The CN from HIV fails to bind to the mutant Vav protein lacking the C-terminal SH3 domain (Vav S3) (lanes 5-8) but interacts with Vav2 (lanes 1-4) in COS cells.	bind
14307	3	4858	5	NULL	NULL	0	NULL	CN	NULL	HIV	interacts with	NULL				Vav2	NULL				NULL	in COS cells	NULL	NULL	NULL	NULL	gw60_molcell_3_6_729_s_58	10394361	(C) The CN from HIV fails to bind to the mutant Vav protein lacking the C-terminal SH3 domain (Vav S3) (lanes 5-8) but interacts with Vav2 (lanes 1-4) in COS cells.	bind
12595	3	4858	6	NULL	NULL	NULL	NULL	CN	GP	HIV	does not bind					Vav S3	GP				NULL	COS cells	NULL	NULL	NULL	NULL	gw60_molcell_3_6_729_s_58	10394361	(C) The CN from HIV fails to bind to the mutant Vav protein lacking the C-terminal SH3 domain (Vav S3) (lanes 5-8) but interacts with Vav2 (lanes 1-4) in COS cells.	bind
12596	2	4858	6	NULL	NULL	NULL	NULL	CN	GP	HIV	interacts with					Vav2	GP				NULL	COS cells	NULL	NULL	NULL	NULL	gw60_molcell_3_6_729_s_58	10394361	(C) The CN from HIV fails to bind to the mutant Vav protein lacking the C-terminal SH3 domain (Vav S3) (lanes 5-8) but interacts with Vav2 (lanes 1-4) in COS cells.	bind
54551	1	4858	6	NULL	NULL	NULL	NULL	Vav S3	GP		is					Vav protein	GP	mutant;;lacking	C-terminal SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_6_729_s_58	10394361	(C) The CN from HIV fails to bind to the mutant Vav protein lacking the C-terminal SH3 domain (Vav S3) (lanes 5-8) but interacts with Vav2 (lanes 1-4) in COS cells.	bind
14308	1	4860	5	NULL	NULL	0	NULL	Sac6	NULL		bind	NULL				actin filaments	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_7_2617_s_253	12857851	(C) The concentrations of Sac6 ( ) and Scp1 ( ) bound to  actin filaments were calculated from gel densitometry and plotted versus  the  total concentration of His6-Scp1 in the reactions.	bind
14309	2	4860	5	NULL	NULL	0	NULL	Scp1	NULL		bind	NULL				actin filaments	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_7_2617_s_253	12857851	(C) The concentrations of Sac6 ( ) and Scp1 ( ) bound to  actin filaments were calculated from gel densitometry and plotted versus  the  total concentration of His6-Scp1 in the reactions.	bind
12597	1	4860	6	NULL	NULL	NULL	NULL	sac6	GP		bind					actin filament	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_7_2617_s_253	12857851	(C) The concentrations of Sac6 ( ) and Scp1 ( ) bound to  actin filaments were calculated from gel densitometry and plotted versus  the  total concentration of His6-Scp1 in the reactions.	bind
12598	2	4860	6	NULL	NULL	NULL	NULL	Scp1	GP		bind					actin filament	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_7_2617_s_253	12857851	(C) The concentrations of Sac6 ( ) and Scp1 ( ) bound to  actin filaments were calculated from gel densitometry and plotted versus  the  total concentration of His6-Scp1 in the reactions.	bind
14310	1	4861	5	NULL	NULL	0	NULL	Sac6	NULL		bind	NULL				actin filaments	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_7_2617_s_253	12857851	(C) The concentrations of Sac6 ( ) and Scp1 ( ) bound to  actin filaments were calculated from gel densitometry and plotted versus the  total concentration of His6-Scp1 in the reactions.	bind
14311	2	4861	5	NULL	NULL	0	NULL	Scp1	NULL		bind	NULL				actin filaments	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_7_2617_s_253	12857851	(C) The concentrations of Sac6 ( ) and Scp1 ( ) bound to  actin filaments were calculated from gel densitometry and plotted versus the  total concentration of His6-Scp1 in the reactions.	bind
14312	1	4862	5	10	NULL	0	NULL	GST-GraudeltaN 			bind			E493K		DNA					NULL		NULL	NULL	NULL	NULL	gw60_genetics_155_4_1831_s_163	10924478	(C) The DNA-binding activity of the GST-GraudeltaN E493K and C298Y fusions was analyzed by gel-shift assay.	bind
14313	2	4862	5	10	NULL	0	NULL	GST-GraudeltaN 			bind			C298Y		DNA					NULL		NULL	NULL	NULL	NULL	gw60_genetics_155_4_1831_s_163	10924478	(C) The DNA-binding activity of the GST-GraudeltaN E493K and C298Y fusions was analyzed by gel-shift assay.	bind
54552	3	4862	5	10	NULL	0	NULL	GST-GraudeltaN			is a type of			E493K		fusion protein					NULL		0	NULL	NULL	NULL	gw60_genetics_155_4_1831_s_163	10924478	(C) The DNA-binding activity of the GST-GraudeltaN E493K and C298Y fusions was analyzed by gel-shift assay.	bind
54553	4	4862	5	10	NULL	0	NULL	GST-GraudeltaN			is a type of			C298Y		fusion protein					NULL		0	NULL	NULL	NULL	gw60_genetics_155_4_1831_s_163	10924478	(C) The DNA-binding activity of the GST-GraudeltaN E493K and C298Y fusions was analyzed by gel-shift assay.	bind
12599	1	4862	6	NULL	NULL	NULL	NULL	GST-GraudeltaN	GP		bind			E493K		DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genetics_155_4_1831_s_163	10924478	(C) The DNA-binding activity of the GST-GraudeltaN E493K and C298Y fusions was analyzed by gel-shift assay.	bind
12821	2	4862	6	NULL	NULL	NULL	NULL	GST-GraudeltaN	GP		bind			C298Y		DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genetics_155_4_1831_s_163	10924478	(C) The DNA-binding activity of the GST-GraudeltaN E493K and C298Y fusions was analyzed by gel-shift assay.	bind
54554	3	4862	6	NULL	NULL	NULL	NULL	GST-GraudeltaN 	GP		is a type of			E493K		fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_genetics_155_4_1831_s_163	10924478	(C) The DNA-binding activity of the GST-GraudeltaN E493K and C298Y fusions was analyzed by gel-shift assay.	bind
54555	4	4862	6	NULL	NULL	NULL	NULL	GST-GraudeltaN	GP		is a type of			 C298Y		fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_genetics_155_4_1831_s_163	10924478	(C) The DNA-binding activity of the GST-GraudeltaN E493K and C298Y fusions was analyzed by gel-shift assay.	bind
16293	1	4863	5	NULL	NULL	0	NULL	annexin V	NULL		bind	NULL				PI	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_173_1_133_s_123	16606695	(C) The duration from  rounding to annexin V binding and annexin V binding to PI uptake was calculated for  individual cells and is presented as means  plus-or-minus  SEM (error bars;  n = 33).	bind
12822	1	4863	6	NULL	NULL	NULL	NULL	annexin V	GP		bind					PI	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_1_133_s_123	16606695	(C) The duration from  rounding to annexin V binding and annexin V binding to PI uptake was calculated for  individual cells and is presented as means  plus-or-minus  SEM (error bars;  n = 33).	bind
14314	1	4866	5	10	NULL	0	NULL	NahR			bind					Psal					NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1725_2_247_s_188	15978733	(C) The effect of salicylate  (0.1, 1 or 10 mM) on the sensorgram of NahR (1  M) binding to  Psal (1000 RU) is shown at a flow rate of 20  l/min.	bind
12614	1	4866	6	NULL	NULL	NULL	NULL	NahR	GP		bind					Psal	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1725_2_247_s_188	15978733	(C) The effect of salicylate  (0.1, 1 or 10 mM) on the sensorgram of NahR (1  M) binding to  Psal (1000 RU) is shown at a flow rate of 20  l/min.	bind
14315	1	4867	5	10	NULL	0	NULL	LPA			induce					IP		generation of			NULL	in HeLa cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_11_5069_s_203	15143197	(C) The effects of  a mutation at the C-terminal PDZ-binding motif of LPA2 on LPA-induced IPs generation in HeLa cells.	bind
12620	1	4867	6	NULL	NULL	NULL	NULL	LPA	Chemical		induces					IP	GP	generation of			NULL	HeLa cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_11_5069_s_203	15143197	(C) The effects of  a mutation at the C-terminal PDZ-binding motif of LPA2 on LPA-induced IPs generation in HeLa cells.	bind
14316	1	4868	5	NULL	NULL	0	NULL	FRL	NULL		bind	NULL		FH1 domain		profilin	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_18_6872_s_269	10958683	(C) The FH1 domain of FRL binds to profilin.	bind
12622	1	4868	6	NULL	NULL	NULL	NULL	FRL	GP		bind			FH1 domain		profilin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_18_6872_s_269	10958683	(C) The FH1 domain of FRL binds to profilin.	bind
14317	1	4869	5	10	NULL	0	NULL	Alp11B			bind		efficiently			alpha-tubulin					NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_9_2987_s_264	10473641	(C) The glycine-rich domain is important for efficient binding between Alp11B and alpha-tubulin.	bind
54556	2	4869	5	10	NULL	0	NULL				is important for			glycine-rich domain		statement 1					NULL		0	NULL	NULL	NULL	gw60_molbiolcell_10_9_2987_s_264	10473641	(C) The glycine-rich domain is important for efficient binding between Alp11B and alpha-tubulin.	bind
12625	1	4869	6	NULL	NULL	NULL	NULL	Alp11B	GP		bind		efficiently			alpha-tubulin	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_9_2987_s_264	10473641	(C) The glycine-rich domain is important for efficient binding between Alp11B and alpha-tubulin.	bind
12627	2	4869	6	NULL	NULL	NULL	NULL				is important for			glycine-rich domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_9_2987_s_264	10473641	(C) The glycine-rich domain is important for efficient binding between Alp11B and alpha-tubulin.	bind
14318	1	4870	5	NULL	NULL	0	NULL	Grp1	NULL		bind	NULL		PH domain		Ins(1,3,4,5)P4	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_8_4_829_s_234	11684018	(C) The Grp1 PH domain bound to Ins(1,3,4,5)P4.	bind
12629	1	4870	6	NULL	NULL	NULL	NULL	Grp1	GP		bind			PH domain		Ins(1,3,4,5)P4	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_4_829_s_234	11684018	(C) The Grp1 PH domain bound to Ins(1,3,4,5)P4.	bind
14319	1	4871	5	NULL	NULL	0	NULL	DdLIMP	NULL		sediments with	NULL				PIP2	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_1_167_s_313	10189376	(C) The highest amount  of DdLIMP is sedimented with PIP2, there is only  minute binding to PC, and moderate binding to  the anionic phospholipid PS.	bind
14320	2	4871	5	10	NULL	0	NULL	DdLIMP			bind					PC					NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_1_167_s_313	10189376	(C) The highest amount  of DdLIMP is sedimented with PIP2, there is only  minute binding to PC, and moderate binding to  the anionic phospholipid PS.	bind
14321	3	4871	5	NULL	NULL	0	NULL	DdLIMP	NULL		bind	NULL	moderate			phospholipid PS	NULL	anionic			NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_1_167_s_313	10189376	(C) The highest amount  of DdLIMP is sedimented with PIP2, there is only  minute binding to PC, and moderate binding to  the anionic phospholipid PS.	bind
12631	1	4871	6	NULL	NULL	NULL	NULL	DdLIMP	GP		bind					PIP2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_1_167_s_313	10189376	(C) The highest amount  of DdLIMP is sedimented with PIP2, there is only  minute binding to PC, and moderate binding to  the anionic phospholipid PS.	bind
12688	2	4871	6	NULL	NULL	NULL	NULL	DdLIMP	GP		bind					PC	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_1_167_s_313	10189376	(C) The highest amount  of DdLIMP is sedimented with PIP2, there is only  minute binding to PC, and moderate binding to  the anionic phospholipid PS.	bind
12689	3	4871	6	NULL	NULL	NULL	NULL	DdLIMP	GP		bind		moderate			phospholipid PS	CellComponent	anionic			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_1_167_s_313	10189376	(C) The highest amount  of DdLIMP is sedimented with PIP2, there is only  minute binding to PC, and moderate binding to  the anionic phospholipid PS.	bind
14322	1	4872	5	NULL	NULL	0	NULL	SMRT	NULL		bind	NULL				RARbeta	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_23_8_2844_s_163	12665583	(C) The I412T mutant enhances SMRT binding by RARbeta, but not RARalpha, in a GST-protein interaction assay in vitro.	bind
14323	2	4872	5	NULL	NULL	0	NULL		NULL	mutant	enhances	NULL		I412T		statement 1	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_23_8_2844_s_163	12665583	(C) The I412T mutant enhances SMRT binding by RARbeta, but not RARalpha, in a GST-protein interaction assay in vitro.	bind
14324	3	4872	5	NULL	NULL	0	NULL	SMRT	NULL		bind	NULL				RARalpha	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_23_8_2844_s_163	12665583	(C) The I412T mutant enhances SMRT binding by RARbeta, but not RARalpha, in a GST-protein interaction assay in vitro.	bind
14325	4	4872	5	NULL	NULL	0	NULL		NULL	mutant	does not enhance	NULL		I412T		statement 3	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_23_8_2844_s_163	12665583	(C) The I412T mutant enhances SMRT binding by RARbeta, but not RARalpha, in a GST-protein interaction assay in vitro.	bind
12690	1	4872	6	NULL	NULL	NULL	NULL	SMRT	GP		bind					RARbeta	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_23_8_2844_s_163	12665583	(C) The I412T mutant enhances SMRT binding by RARbeta, but not RARalpha, in a GST-protein interaction assay in vitro.	bind
12691	2	4872	6	NULL	NULL	NULL	NULL	SMRT	GP		bind					RARalpha	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_23_8_2844_s_163	12665583	(C) The I412T mutant enhances SMRT binding by RARbeta, but not RARalpha, in a GST-protein interaction assay in vitro.	bind
12692	3	4872	6	NULL	NULL	NULL	NULL			mutant	enhances			I412T		statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_23_8_2844_s_163	12665583	(C) The I412T mutant enhances SMRT binding by RARbeta, but not RARalpha, in a GST-protein interaction assay in vitro.	bind
12693	4	4872	6	NULL	NULL	NULL	NULL			mutant	does not enhance			I412T		statement 2	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_23_8_2844_s_163	12665583	(C) The I412T mutant enhances SMRT binding by RARbeta, but not RARalpha, in a GST-protein interaction assay in vitro.	bind
14326	1	4873	5	NULL	NULL	0	NULL	HIF-1	NULL		bind	NULL				PSMA7	NULL				NULL	in vivo	0	NULL	NULL	NULL	gw60_febslett_498_1_62_s_82	11389899	(C) The in vivo binding of HIF-1  to PSMA7 was confirmed by co-immunoprecipitation.	bind
12694	1	4873	6	NULL	NULL	NULL	NULL	HIF-1	GP		bind					PSMA7	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_febslett_498_1_62_s_82	11389899	(C) The in vivo binding of HIF-1  to PSMA7 was confirmed by co-immunoprecipitation.	bind
14327	1	4874	5	NULL	NULL	0	NULL	Chl4p	NULL		interacts with	NULL				CEN DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_2_460_s_108	12589047	(C) The interaction of Chl4p with  CEN DNA depends on Ctf19p.	bind
14328	2	4874	5	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				Ctf19p	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_2_460_s_108	12589047	(C) The interaction of Chl4p with  CEN DNA depends on Ctf19p.	bind
12695	1	4874	6	NULL	NULL	NULL	NULL	Chl4p	GP		interacts with					CEN DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_2_460_s_108	12589047	(C) The interaction of Chl4p with  CEN DNA depends on Ctf19p.	bind
12696	2	4874	6	NULL	NULL	NULL	NULL	statement 1	Process		is dependent on					Ctf19p	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_2_460_s_108	12589047	(C) The interaction of Chl4p with  CEN DNA depends on Ctf19p.	bind
14329	1	4875	5	NULL	NULL	0	NULL	nm23-H2	NULL	kinase negative mutant 	bind	NULL				Lbc	NULL	mutant	H118F		NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_4_1063_s_98	15249197	(C) The kinase negative  mutant of nm23-H2 binds to Lbc. H118F mutant was expressed and subjected to binding  assay.	bind
12697	1	4875	6	NULL	NULL	NULL	NULL	nm23-H2		kinase negative mutant	bind					Lbc	GP	mutant	H118F		NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_4_1063_s_98	15249197	(C) The kinase negative  mutant of nm23-H2 binds to Lbc. H118F mutant was expressed and subjected to binding  assay.	bind
14330	1	4876	5	10	NULL	0	NULL	nucleosomes 			does not bind				last 13 bp of DNA	histone octamer					NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_22_10047_s_124	15509805	(c) The last 13 bp of DNA on nucleosomes slid by ISW2 were not bound to the histone  octamer, as shown by exonuclease III footprinting.	bind
12699	2	4876	6	NULL	NULL	NULL	NULL	nucleosomes			does not bind				last 13 bp of DNA on	histone octamer					NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_22_10047_s_124	15509805	(c) The last 13 bp of DNA on nucleosomes slid by ISW2 were not bound to the histone  octamer, as shown by exonuclease III footprinting.	bind
14331	1	4877	5	NULL	NULL	0	NULL	Nyv1p	NULL		bind	NULL		longin domain		AP3	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw70_molbiolcell_17_10_4282_s_291	16855025	(C) The longin domain of Nyv1p binds to  AP3 in vitro.	bind
12700	1	4877	6	NULL	NULL	NULL	NULL	Nyv1p	GP		bind			longin domain		AP3	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molbiolcell_17_10_4282_s_291	16855025	(C) The longin domain of Nyv1p binds to  AP3 in vitro.	bind
14332	1	4878	5	NULL	NULL	0	NULL	G-CSF	NULL	biotin-labeled	bind	NULL				G-CSF receptor	NULL				NULL	UT-7/GR cell surface	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_319_2_582_s_145	15178446	(C) The mean fluorescence  intensity (MFI) that represents biotin-labeled G-CSF bound to G-CSF receptor expressed  on the UT-7/GR cell surface was competitively suppressed by G-CSF-PE40 in a dose-dependent  manner.	bind
14333	2	4878	5	10	NULL	0	NULL	G-CSF-PE40			supress		competitively;;dose dependently			statement 1					NULL	UT-7/GR cell surface	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_319_2_582_s_145	15178446	(C) The mean fluorescence  intensity (MFI) that represents biotin-labeled G-CSF bound to G-CSF receptor expressed  on the UT-7/GR cell surface was competitively suppressed by G-CSF-PE40 in a dose-dependent  manner.	bind
12823	1	4878	6	NULL	NULL	NULL	NULL	G-CSF	GP	biotin-labeled	bind					G-CSF receptor	GP				NULL	UT-7/GR cell surface	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_319_2_582_s_145	15178446	(C) The mean fluorescence  intensity (MFI) that represents biotin-labeled G-CSF bound to G-CSF receptor expressed  on the UT-7/GR cell surface was competitively suppressed by G-CSF-PE40 in a dose-dependent  manner.	bind
12824	2	4878	6	NULL	NULL	NULL	NULL	G-CSF-PE40	GP		suppresses		competitively;;dose dependently			statement 1	Process				NULL	UT-7/GR cell surface	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_319_2_582_s_145	15178446	(C) The mean fluorescence  intensity (MFI) that represents biotin-labeled G-CSF bound to G-CSF receptor expressed  on the UT-7/GR cell surface was competitively suppressed by G-CSF-PE40 in a dose-dependent  manner.	bind
14334	1	4879	5	NULL	NULL	0	NULL	Msb3	NULL		bind	NULL		N-terminal non-GAP region		Spa2	NULL		SHD-I region		NULL	in vitro	0	NULL	NULL	NULL	gw70_molcellbiol_25_19_8567_s_40	16166638	(C) The N-terminal, non-GAP  region of Msb3 or Msb4 binds to the SHD-I region of Spa2 in vitro.	bind
14335	2	4879	5	NULL	NULL	0	NULL	Msb4	NULL		bind	NULL		N-terminal non-GAP region		Spa2	NULL		SHD-I region		NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8567_s_40	16166638	(C) The N-terminal, non-GAP  region of Msb3 or Msb4 binds to the SHD-I region of Spa2 in vitro.	bind
14336	3	4879	5	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_19_8567_s_40	16166638	(C) The N-terminal, non-GAP  region of Msb3 or Msb4 binds to the SHD-I region of Spa2 in vitro.	bind
12716	1	4879	6	NULL	NULL	NULL	NULL	Msb3	GP		bind			N-terminal non-GAP region		Spa2	GP		SHD-I		NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8567_s_40	16166638	(C) The N-terminal, non-GAP  region of Msb3 or Msb4 binds to the SHD-I region of Spa2 in vitro.	bind
12717	2	4879	6	NULL	NULL	NULL	NULL	Msb4	GP		bind			N-terminal non-GAP region		Spa2	GP		SHD-I		NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8567_s_40	16166638	(C) The N-terminal, non-GAP  region of Msb3 or Msb4 binds to the SHD-I region of Spa2 in vitro.	bind
12718	3	4879	6	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8567_s_40	16166638	(C) The N-terminal, non-GAP  region of Msb3 or Msb4 binds to the SHD-I region of Spa2 in vitro.	bind
14337	1	4880	5	NULL	NULL	0	NULL	anti-Nischarin antibody	NULL	chicken	bind	NULL				Nischarin	NULL	endogenous			NULL	in RIE cells	0	NULL	NULL	NULL	gw60_cellbiol_151_6_1141_s_265	11121431	(C) The peptide used for immunization can block the binding of chicken anti-Nischarin antibody both to endogenous Nischarin in RIE cells and to expressed Nischarin in Cos7 cells.	bind
14339	2	4880	5	10	NULL	0	NULL	anti-Nischarin antibody	NULL	chicken	bind	NULL				Nischarin 	NULL				NULL	expressed in Cos7 cells	NULL	NULL	NULL	NULL	gw60_cellbiol_151_6_1141_s_265	11121431	(C) The peptide used for immunization can block the binding of chicken anti-Nischarin antibody both to endogenous Nischarin in RIE cells and to expressed Nischarin in Cos7 cells.	bind
12719	1	4880	6	NULL	NULL	NULL	NULL	anti-Nischarin antibody	GP	chicken	bind					Nischarin	GP	endogenous			NULL	RIE cells	NULL	NULL	NULL	NULL	gw60_cellbiol_151_6_1141_s_265	11121431	(C) The peptide used for immunization can block the binding of chicken anti-Nischarin antibody both to endogenous Nischarin in RIE cells and to expressed Nischarin in Cos7 cells.	bind
12720	2	4880	6	NULL	NULL	NULL	NULL	anti-Nischarin antibody	GP	chicken	bind					Nischarin	GP				NULL	expressed in Cos7 cells	NULL	NULL	NULL	NULL	gw60_cellbiol_151_6_1141_s_265	11121431	(C) The peptide used for immunization can block the binding of chicken anti-Nischarin antibody both to endogenous Nischarin in RIE cells and to expressed Nischarin in Cos7 cells.	bind
14418	1	4881	5	NULL	NULL	0	NULL	PPT1	NULL	bovine	bind	NULL				palmitate	NULL				NULL		0	NULL	NULL	NULL	gw60_gene_312_0_271_s_96	12909364	(C) The predicted amino acid sequence of CG12108 and human PPT1 were superimposed onto the crystal structure of bovine PPT1 bound to palmitate (PDB#1EH5) using MSA-3D, and the results viewed using Protein Explorer.	bind
12722	1	4881	6	NULL	NULL	NULL	NULL	PPT1	GP	bovine	bind					palmitate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_gene_312_0_271_s_96	12909364	(C) The predicted amino acid sequence of CG12108 and human PPT1 were superimposed onto the crystal structure of bovine PPT1 bound to palmitate (PDB#1EH5) using MSA-3D, and the results viewed using Protein Explorer.	bind
14419	1	4884	5	NULL	NULL	0	NULL	GTP S	NULL		bind	NULL				myr-yARF2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_3_3_275_s_128	10198630	(C) The Sec7 domain of yeast Gea1p (wild type) or the same domain carrying the mutation M699L was purified from  E. coli and tested for stimulation of GTP S binding to myr-yARF2 in the presence or absence of BFA.	bind
12723	1	4884	6	NULL	NULL	NULL	NULL	GTP S	Chemical		bind					myr-yARF2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_3_275_s_128	10198630	(C) The Sec7 domain of yeast Gea1p (wild type) or the same domain carrying the mutation M699L was purified from  E. coli and tested for stimulation of GTP S binding to myr-yARF2 in the presence or absence of BFA.	bind
14420	1	4885	5	NULL	NULL	0	NULL	BiP	NULL		bind	NULL				HC	NULL				NULL		0	NULL	NULL	NULL	gw60_immunity_15_1_105_s_227	11485742	(C) The signals for HC and labeled BiP were quantitated by densiotometry, and the relative amount of BiP bound to HC was determined with the value at 150 min set to 100	bind
12724	1	4885	6	NULL	NULL	NULL	NULL	BiP	GP		bind					HC	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_15_1_105_s_227	11485742	(C) The signals for HC and labeled BiP were quantitated by densiotometry, and the relative amount of BiP bound to HC was determined with the value at 150 min set to 100	bind
14421	1	4886	5	NULL	NULL	0	NULL	TopBP1	NULL		bind	NULL		sixth BRCT domain		E2F1	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_9_3287_s_167	12697828	(C) The sixth BRCT domain of TopBP1  binds E2F1.	bind
12725	1	4886	6	NULL	NULL	NULL	NULL	TopBP1	GP		bind			sixth BRCT domain		E2F1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_9_3287_s_167	12697828	(C) The sixth BRCT domain of TopBP1  binds E2F1.	bind
14422	1	4888	5	NULL	NULL	0	NULL	Sox-2	NULL		bind	NULL				UTF1	NULL			regulatory element	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_8_5453_s_219	10409735	(C) The Sox-2 and chimera 1 bearing the POU DNA binding domain of Oct-6 bind to the UTF1 regulatory element in a mutually exclusive manner.	bind
14423	2	4888	5	NULL	NULL	0	NULL	chimera 1	NULL		bind	NULL		POU DNA binding domain of Oct-6		UTF1	NULL			regulatory element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5453_s_219	10409735	(C) The Sox-2 and chimera 1 bearing the POU DNA binding domain of Oct-6 bind to the UTF1 regulatory element in a mutually exclusive manner.	bind
14424	3	4888	5	NULL	NULL	0	NULL	statement 1	NULL		mutually exclusive to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_8_5453_s_219	10409735	(C) The Sox-2 and chimera 1 bearing the POU DNA binding domain of Oct-6 bind to the UTF1 regulatory element in a mutually exclusive manner.	bind
12726	1	4888	6	NULL	NULL	NULL	NULL	Sox-2	GP		bind					UTF-1	GP			regulatory element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5453_s_219	10409735	(C) The Sox-2 and chimera 1 bearing the POU DNA binding domain of Oct-6 bind to the UTF1 regulatory element in a mutually exclusive manner.	bind
12727	2	4888	6	NULL	NULL	NULL	NULL	chimera 1	GP		bind			POU DNA binding domain of Oct-6		UTF-1	GP			regulatory element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5453_s_219	10409735	(C) The Sox-2 and chimera 1 bearing the POU DNA binding domain of Oct-6 bind to the UTF1 regulatory element in a mutually exclusive manner.	bind
12728	3	4888	6	NULL	NULL	NULL	NULL	statement 1	Process		is independent of					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5453_s_219	10409735	(C) The Sox-2 and chimera 1 bearing the POU DNA binding domain of Oct-6 bind to the UTF1 regulatory element in a mutually exclusive manner.	bind
14425	1	4889	5	NULL	NULL	0	NULL	GBD hybrid	NULL		bind	NULL					NULL			Gal4 binding sites	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_23_8292_s_125	12417731	(C) The strain is the same as in panel B except that a GBD hybrid binds to the Gal4 binding sites and causes silencing of the  URA3 gene.	bind
14426	2	4889	5	NULL	NULL	0	NULL	statement 1	NULL		causes	NULL				URA3 gene	NULL	silencing of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_23_8292_s_125	12417731	(C) The strain is the same as in panel B except that a GBD hybrid binds to the Gal4 binding sites and causes silencing of the  URA3 gene.	bind
12729	1	4889	6	NULL	NULL	NULL	NULL	GBD hybrid			bind									Gal4 binding sites	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_23_8292_s_125	12417731	(C) The strain is the same as in panel B except that a GBD hybrid binds to the Gal4 binding sites and causes silencing of the  URA3 gene.	bind
12730	2	4889	6	NULL	NULL	NULL	NULL	statement 1			causes					URA3 gene	GP	silencing of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_23_8292_s_125	12417731	(C) The strain is the same as in panel B except that a GBD hybrid binds to the Gal4 binding sites and causes silencing of the  URA3 gene.	bind
14417	2	4890	5	10	NULL	0	NULL	Ras		distal	bind					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_cell_112_5_685_s_33	12628188	(C) The structure of the distal Ras bound to the GTP analog GppNp from the RasY64A complex is shown on the left (structure D).	bind
54557	1	4890	5	10	NULL	0	NULL	GppNp 			is from					RasY64A complex					NULL		0	NULL	NULL	NULL	gw60_cell_112_5_685_s_33	12628188	(C) The structure of the distal Ras bound to the GTP analog GppNp from the RasY64A complex is shown on the left (structure D).	bind
54558	3	4890	5	10	NULL	0	NULL	GppNp			is a type of					GTP analog					NULL		0	NULL	NULL	NULL	gw60_cell_112_5_685_s_33	12628188	(C) The structure of the distal Ras bound to the GTP analog GppNp from the RasY64A complex is shown on the left (structure D).	bind
12731	1	4890	6	NULL	NULL	NULL	NULL	GppNp	Chemical		is from					Ras complex	GP		Y64A		NULL		NULL	NULL	NULL	NULL	gw60_cell_112_5_685_s_33	12628188	(C) The structure of the distal Ras bound to the GTP analog GppNp from the RasY64A complex is shown on the left (structure D).	bind
12732	2	4890	6	NULL	NULL	NULL	NULL	Ras	GP	distal	bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_5_685_s_33	12628188	(C) The structure of the distal Ras bound to the GTP analog GppNp from the RasY64A complex is shown on the left (structure D).	bind
41696	3	4890	6	NULL	NULL	NULL	NULL	GppNp	Chemical		is a type of					GTP analog	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_5_685_s_33	12628188	(C) The structure of the distal Ras bound to the GTP analog GppNp from the RasY64A complex is shown on the left (structure D).	bind
14427	1	4891	5	NULL	NULL	0	NULL	DinR	NULL		bind	NULL				dinR	NULL			promoter/operator	NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_8_2201_s_227	9555905	(C) Three-dimensional representation of the bases within the  recA operator that are protected by DinR during hydroxyl radical cleavage, indicating that the protected sites lie on one face of [[ the DNA.                     The nondenaturing gel mobility shift assay ]] suggests that DinR apparently binds to the  dinR promoter/operator to form two major protein-DNA species (Fig.  5).	bind
14428	2	4891	5	10	NULL	0	NULL	statement 1			forms					 protein-DNA species		two major			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_8_2201_s_227	9555905	(C) Three-dimensional representation of the bases within the  recA operator that are protected by DinR during hydroxyl radical cleavage, indicating that the protected sites lie on one face of [[ the DNA.                     The nondenaturing gel mobility shift assay ]] suggests that DinR apparently binds to the  dinR promoter/operator to form two major protein-DNA species (Fig.  5).	bind
16294	3	4891	5	NULL	NULL	0	NULL	recA	NULL		protected by	NULL			operator	DinR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_8_2201_s_227	9555905	(C) Three-dimensional representation of the bases within the  recA operator that are protected by DinR during hydroxyl radical cleavage, indicating that the protected sites lie on one face of [[ the DNA.                     The nondenaturing gel mobility shift assay ]] suggests that DinR apparently binds to the  dinR promoter/operator to form two major protein-DNA species (Fig.  5).	bind
16295	4	4891	5	NULL	NULL	0	NULL	statement 3	NULL		occurs during	NULL				hydroxyl radical cleavage	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_8_2201_s_227	9555905	(C) Three-dimensional representation of the bases within the  recA operator that are protected by DinR during hydroxyl radical cleavage, indicating that the protected sites lie on one face of [[ the DNA.                     The nondenaturing gel mobility shift assay ]] suggests that DinR apparently binds to the  dinR promoter/operator to form two major protein-DNA species (Fig.  5).	bind
12733	1	4891	6	NULL	NULL	NULL	NULL	DinR	GP		bind					dinR	GP			promoter/operator	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_8_2201_s_227	9555905	(C) Three-dimensional representation of the bases within the  recA operator that are protected by DinR during hydroxyl radical cleavage, indicating that the protected sites lie on one face of [[ the DNA.                     The nondenaturing gel mobility shift assay ]] suggests that DinR apparently binds to the  dinR promoter/operator to form two major protein-DNA species (Fig.  5).	bind
12734	2	4891	6	NULL	NULL	NULL	NULL	recA	GP		protected by				operator	DinR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_8_2201_s_227	9555905	(C) Three-dimensional representation of the bases within the  recA operator that are protected by DinR during hydroxyl radical cleavage, indicating that the protected sites lie on one face of [[ the DNA.                     The nondenaturing gel mobility shift assay ]] suggests that DinR apparently binds to the  dinR promoter/operator to form two major protein-DNA species (Fig.  5).	bind
12735	3	4891	6	NULL	NULL	NULL	NULL	statement 2	Process		occurs during					hydroxyl radical cleavage	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_8_2201_s_227	9555905	(C) Three-dimensional representation of the bases within the  recA operator that are protected by DinR during hydroxyl radical cleavage, indicating that the protected sites lie on one face of [[ the DNA.                     The nondenaturing gel mobility shift assay ]] suggests that DinR apparently binds to the  dinR promoter/operator to form two major protein-DNA species (Fig.  5).	bind
16300	4	4891	6	NULL	NULL	NULL	NULL	statement 1	Process		forms					protein-DNA species		two major			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_8_2201_s_227	9555905	(C) Three-dimensional representation of the bases within the  recA operator that are protected by DinR during hydroxyl radical cleavage, indicating that the protected sites lie on one face of [[ the DNA.                     The nondenaturing gel mobility shift assay ]] suggests that DinR apparently binds to the  dinR promoter/operator to form two major protein-DNA species (Fig.  5).	bind
14429	1	4892	5	NULL	NULL	0	NULL	GTP S	NULL		bind	NULL				ARF6-His	NULL				NULL		NULL	NULL	NULL	NULL	gw70_febslett_579_2_343_s_34	15642342	(C) Time course of [35]GTP S binding to ARF6-His.	bind
12736	1	4892	6	NULL	NULL	NULL	NULL	GTP S	Chemical		bind					ARF6-His	GP				NULL		NULL	NULL	NULL	NULL	gw70_febslett_579_2_343_s_34	15642342	(C) Time course of [35]GTP S binding to ARF6-His.	bind
14430	1	4893	5	NULL	NULL	0	NULL	collagen	NULL		bind	NULL					NULL		upper front edge of I domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_101_1_47_s_95	10778855	(C) Top view of complex, showing how collagen  binds to the upper front edge of the I domain.	bind
12737	1	4893	6	NULL	NULL	NULL	NULL	collagen	GP		bind								upper front edge of the I domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_101_1_47_s_95	10778855	(C) Top view of complex, showing how collagen  binds to the upper front edge of the I domain.	bind
14431	1	4895	5	NULL	NULL	0	NULL	TR	NULL		bind	NULL				TRAP220	NULL	deletion mutants containing one or both	LXXLL motifs		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_153	10891484	(C) TR binds only TRAP220 deletion mutants containing one or both of the LXXLL motifs.	bind
12738	1	4895	6	NULL	NULL	NULL	NULL	TR	GP		bind					TRAP220	GP	deletion mutants	LXXLL motifs		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_153	10891484	(C) TR binds only TRAP220 deletion mutants containing one or both of the LXXLL motifs.	bind
14432	2	4896	5	10	NULL	0	NULL	CD40		mutant	does not bind		directly			TRAF6					NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9806_s_298	16260598	(C) TRAF6 and TRAF2 coimmunoprecipitate  in CD40L-stimulated carcinoma cells carrying a mutated CD40 that does not directly  bind TRAF6.	bind
44576	1	4896	5	10	NULL	0	NULL	TRAF6			bind					TRAF2					NULL	CD40L-stimulated carcinoma cells carrying a mutated CD40	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9806_s_298	16260598	(C) TRAF6 and TRAF2 coimmunoprecipitate  in CD40L-stimulated carcinoma cells carrying a mutated CD40 that does not directly  bind TRAF6.	bind
12739	1	4896	6	NULL	NULL	NULL	NULL	TRAF6	GP		bind					TRAF2	GP				NULL	CD40L-stimulated carcinoma cells carrying a mutated CD40	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9806_s_298	16260598	(C) TRAF6 and TRAF2 coimmunoprecipitate  in CD40L-stimulated carcinoma cells carrying a mutated CD40 that does not directly  bind TRAF6.	bind
12740	2	4896	6	NULL	NULL	NULL	NULL	CD40	GP	mutant	does not bind		directly			TRAF6	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9806_s_298	16260598	(C) TRAF6 and TRAF2 coimmunoprecipitate  in CD40L-stimulated carcinoma cells carrying a mutated CD40 that does not directly  bind TRAF6.	bind
14437	1	4897	5	NULL	NULL	0	NULL	Raf	NULL		induce	NULL				mdm2	NULL	transcription of			NULL		0	NULL	NULL	NULL	gw60_cell_103_2_321_s_49	11057904	(C) Transcriptional induction of  mdm2 by Raf is independent of p53.	bind
14438	2	4897	5	NULL	NULL	0	NULL	statement 1	NULL		is independent of	NULL				p53	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_103_2_321_s_49	11057904	(C) Transcriptional induction of  mdm2 by Raf is independent of p53.	bind
12788	1	4897	6	NULL	NULL	NULL	NULL	Raf	GP		induces		transcriptionally			mdm2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_2_321_s_49	11057904	(C) Transcriptional induction of  mdm2 by Raf is independent of p53.	bind
12789	2	4897	6	NULL	NULL	NULL	NULL	statement 1	Process		is independent of					p53	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_2_321_s_49	11057904	(C) Transcriptional induction of  mdm2 by Raf is independent of p53.	bind
14439	1	4898	5	NULL	NULL	0	NULL	C2C12 nuclear proteins	NULL		bind	NULL				MEF-1 oligodeoxynucleotide	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_316	11940648	(C) Transfection of a Flag-Id2 expression plasmid inhibits the binding of C2C12 nuclear proteins to the MEF-1 oligodeoxynucleotide, and induced p204 overcomes the inhibition.	bind
14440	2	4898	5	10	NULL	0	NULL	Flag-Id2 expression plasmid			inhibit					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_316	11940648	(C) Transfection of a Flag-Id2 expression plasmid inhibits the binding of C2C12 nuclear proteins to the MEF-1 oligodeoxynucleotide, and induced p204 overcomes the inhibition.	bind
14441	3	4898	5	NULL	NULL	0	NULL	p204	NULL	induced	overcomes	NULL				statement 1	NULL	inhibition of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_316	11940648	(C) Transfection of a Flag-Id2 expression plasmid inhibits the binding of C2C12 nuclear proteins to the MEF-1 oligodeoxynucleotide, and induced p204 overcomes the inhibition.	bind
12790	1	4898	6	NULL	NULL	NULL	NULL	C2C12 nuclear proteins	GP		bind					MEF-1 oligodeoxynucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_316	11940648	(C) Transfection of a Flag-Id2 expression plasmid inhibits the binding of C2C12 nuclear proteins to the MEF-1 oligodeoxynucleotide, and induced p204 overcomes the inhibition.	bind
12791	2	4898	6	NULL	NULL	NULL	NULL	Flag-Id2 expression plasmid 			inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_316	11940648	(C) Transfection of a Flag-Id2 expression plasmid inhibits the binding of C2C12 nuclear proteins to the MEF-1 oligodeoxynucleotide, and induced p204 overcomes the inhibition.	bind
12792	3	4898	6	NULL	NULL	NULL	NULL	p204	GP	induced	overcomes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_316	11940648	(C) Transfection of a Flag-Id2 expression plasmid inhibits the binding of C2C12 nuclear proteins to the MEF-1 oligodeoxynucleotide, and induced p204 overcomes the inhibition.	bind
14442	1	4899	5	NULL	NULL	0	NULL	mant-ADP	NULL		bind	NULL				PI3K	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_103_6_931_s_120	11136978	(C) Transient and steady-state  measurements of mant-ATP and mant-ADP binding to PI3K.	bind
14443	2	4899	5	NULL	NULL	0	NULL	mant-ATP	NULL		bind	NULL				PI3K	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_103_6_931_s_120	11136978	(C) Transient and steady-state  measurements of mant-ATP and mant-ADP binding to PI3K.	bind
12793	1	4899	6	NULL	NULL	NULL	NULL	mant-ATP	Chemical		bind					PI3K	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_6_931_s_120	11136978	(C) Transient and steady-state  measurements of mant-ATP and mant-ADP binding to PI3K.	bind
12794	2	4899	6	NULL	NULL	NULL	NULL	mant-ADP	Chemical		bind					PI3K	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_6_931_s_120	11136978	(C) Transient and steady-state  measurements of mant-ATP and mant-ADP binding to PI3K.	bind
14444	1	4900	5	NULL	NULL	0	NULL	SUV39H1	NULL		bind	NULL				HP1alpha	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw70_molcellbiol_25_7_2525_s_354	15767660	(C) TSA did not affect the in vitro binding of SUV39H1  to HP1alpha as determined by GST pull-down assay.	bind
14445	2	4900	5	NULL	NULL	0	NULL	TSA	NULL		does not affect	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_7_2525_s_354	15767660	(C) TSA did not affect the in vitro binding of SUV39H1  to HP1alpha as determined by GST pull-down assay.	bind
12795	1	4900	6	NULL	NULL	NULL	NULL	SUV39H1	GP		bind					HP1alpha	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_7_2525_s_354	15767660	(C) TSA did not affect the in vitro binding of SUV39H1  to HP1alpha as determined by GST pull-down assay.	bind
12796	2	4900	6	NULL	NULL	NULL	NULL	TSA	Chemical		did not affect					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_7_2525_s_354	15767660	(C) TSA did not affect the in vitro binding of SUV39H1  to HP1alpha as determined by GST pull-down assay.	bind
14446	1	4902	5	NULL	NULL	0	NULL	snapin	NULL	unphosphorylated	bind	NULL				cypin	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_11_5103_s_341	16120643	(C) Unphosphorylated snapin binds to cypin better  than a phosphomimetic form of snapin.	bind
14447	2	4902	5	NULL	NULL	0	NULL	snapin	NULL	phosphomimetic form of	bind	NULL				cypin	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_11_5103_s_341	16120643	(C) Unphosphorylated snapin binds to cypin better  than a phosphomimetic form of snapin.	bind
14448	3	4902	5	NULL	NULL	0	NULL	statement 1	NULL		better than	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_11_5103_s_341	16120643	(C) Unphosphorylated snapin binds to cypin better  than a phosphomimetic form of snapin.	bind
12797	1	4902	6	NULL	NULL	NULL	NULL	snapin	GP	unphosphorylated	bind					cypin	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_11_5103_s_341	16120643	(C) Unphosphorylated snapin binds to cypin better  than a phosphomimetic form of snapin.	bind
12798	2	4902	6	NULL	NULL	NULL	NULL	snapin	GP	phosphomimetic form of	bind					cypin	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_11_5103_s_341	16120643	(C) Unphosphorylated snapin binds to cypin better  than a phosphomimetic form of snapin.	bind
12799	3	4902	6	NULL	NULL	NULL	NULL	statement 1	Process		is better than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_11_5103_s_341	16120643	(C) Unphosphorylated snapin binds to cypin better  than a phosphomimetic form of snapin.	bind
14449	1	4903	5	NULL	NULL	0	NULL	TM-1	NULL	untagged	bind	NULL				Enigma	NULL		PDZ domain		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_6_1973_s_136	10359609	(C) Untagged TM-1 binds to the PDZ domain of Enigma to the same extent as the corresponding fusion protein.	bind
12800	1	4903	6	NULL	NULL	NULL	NULL	TM-1	GP	untagged	bind					Enigma	GP		PDZ domain		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_6_1973_s_136	10359609	(C) Untagged TM-1 binds to the PDZ domain of Enigma to the same extent as the corresponding fusion protein.	bind
14450	1	4904	5	10	NULL	0	NULL	Bru			bind		specifically			grk				3 UTR	NULL		NULL	NULL	NULL	NULL	gw70_mechdev_120_3_289_s_152	12591598	(C) UV cross-linking  RNA competition experiment showing that Bru binds the 3  portion of the  grk 3 UTR specifically.	bind
12801	1	4904	6	NULL	NULL	NULL	NULL	Bru	GP		bind		specifically			grk	GP			3 UTR	NULL		NULL	NULL	NULL	NULL	gw70_mechdev_120_3_289_s_152	12591598	(C) UV cross-linking  RNA competition experiment showing that Bru binds the 3  portion of the  grk 3 UTR specifically.	bind
14451	1	4905	5	NULL	NULL	0	NULL	PTB	NULL		bind	NULL				Sec RNA	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_19_7388_s_266	10982855	(C) UV cross-linking and competition experiments demonstrated that PTB binding to the Sec RNA can be competed using self-competition or using a cold ISS1 competitor.	bind
14452	2	4905	5	10	NULL	0	NULL	 ISS1		cold	bind					Sec RNA					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7388_s_266	10982855	(C) UV cross-linking and competition experiments demonstrated that PTB binding to the Sec RNA can be competed using self-competition or using a cold ISS1 competitor.	bind
14453	3	4905	5	10	NULL	0	NULL	statement 1			compete with					statement 2					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7388_s_266	10982855	(C) UV cross-linking and competition experiments demonstrated that PTB binding to the Sec RNA can be competed using self-competition or using a cold ISS1 competitor.	bind
16296	4	4905	5	NULL	NULL	0	NULL	Sec RNA	NULL		bind	NULL				Sec RNA	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_19_7388_s_266	10982855	(C) UV cross-linking and competition experiments demonstrated that PTB binding to the Sec RNA can be competed using self-competition or using a cold ISS1 competitor.	bind
16297	5	4905	5	NULL	NULL	0	NULL	statement 4	NULL		competes with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_19_7388_s_266	10982855	(C) UV cross-linking and competition experiments demonstrated that PTB binding to the Sec RNA can be competed using self-competition or using a cold ISS1 competitor.	bind
16298	6	4905	5	NULL	NULL	0	NULL	statement 3	NULL		is an alternative to	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_19_7388_s_266	10982855	(C) UV cross-linking and competition experiments demonstrated that PTB binding to the Sec RNA can be competed using self-competition or using a cold ISS1 competitor.	bind
12802	1	4905	6	NULL	NULL	NULL	NULL	PTB	GP		bind					Sec RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7388_s_266	10982855	(C) UV cross-linking and competition experiments demonstrated that PTB binding to the Sec RNA can be competed using self-competition or using a cold ISS1 competitor.	bind
12803	2	4905	6	NULL	NULL	NULL	NULL	 ISS1	GP	cold	bind					Sec RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7388_s_266	10982855	(C) UV cross-linking and competition experiments demonstrated that PTB binding to the Sec RNA can be competed using self-competition or using a cold ISS1 competitor.	bind
12804	3	4905	6	NULL	NULL	NULL	NULL	statement 1	Process		competes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7388_s_266	10982855	(C) UV cross-linking and competition experiments demonstrated that PTB binding to the Sec RNA can be competed using self-competition or using a cold ISS1 competitor.	bind
12805	4	4905	6	NULL	NULL	NULL	NULL	Sec RNA	NucleicAcid		bind					Sec RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7388_s_266	10982855	(C) UV cross-linking and competition experiments demonstrated that PTB binding to the Sec RNA can be competed using self-competition or using a cold ISS1 competitor.	bind
12806	5	4905	6	NULL	NULL	NULL	NULL	statement 1	Process		competes					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7388_s_266	10982855	(C) UV cross-linking and competition experiments demonstrated that PTB binding to the Sec RNA can be competed using self-competition or using a cold ISS1 competitor.	bind
12807	6	4905	6	NULL	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7388_s_266	10982855	(C) UV cross-linking and competition experiments demonstrated that PTB binding to the Sec RNA can be competed using self-competition or using a cold ISS1 competitor.	bind
14454	1	4906	5	NULL	NULL	0	NULL	VRI	NULL		bind	NULL				cry	NULL			E4BP4-consensus sites in promoter	NULL		0	NULL	NULL	NULL	gw60_neuron_37_2_249_s_190	12546820	(C) VRI binds E4BP4-consensus sites in the  cry promoter.	bind
12808	1	4906	6	NULL	NULL	NULL	NULL	VRI	GP		bind					cry	GP			E4BP4-consensus site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_neuron_37_2_249_s_190	12546820	(C) VRI binds E4BP4-consensus sites in the  cry promoter.	bind
14455	2	4907	5	NULL	NULL	0	NULL	Vsm1	NULL		bind	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_8_3114_s_198	12925750	(C) Vsm1 binds to Sso that is not assembled into  SNARE complexes.	bind
44577	1	4907	5	10	NULL	0	NULL	Sso	NULL		is not assembled into	NULL				SNARE complexes	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_8_3114_s_198	12925750	(C) Vsm1 binds to Sso that is not assembled into  SNARE complexes.	bind
12809	1	4907	6	NULL	NULL	NULL	NULL	Sso	GP		is not assembled into					SNARE complexes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_8_3114_s_198	12925750	(C) Vsm1 binds to Sso that is not assembled into  SNARE complexes.	bind
12810	2	4907	6	NULL	NULL	NULL	NULL	Vsm1	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_8_3114_s_198	12925750	(C) Vsm1 binds to Sso that is not assembled into  SNARE complexes.	bind
14456	1	4908	5	NULL	NULL	0	NULL	Sec9	NULL		bind	NULL				Sso1	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_8_3114_s_75	12925750	(C) Vsm1 displaces Sec9 binding to Sso1.	bind
14457	2	4908	5	NULL	NULL	0	NULL	Vsm1	NULL		bind	NULL				Sso1	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_8_3114_s_75	12925750	(C) Vsm1 displaces Sec9 binding to Sso1.	bind
14458	3	4908	5	NULL	NULL	0	NULL	statement 2	NULL		displaces	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_8_3114_s_75	12925750	(C) Vsm1 displaces Sec9 binding to Sso1.	bind
12811	1	4908	6	NULL	NULL	NULL	NULL	Sec9	GP		bind					Sso1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_8_3114_s_75	12925750	(C) Vsm1 displaces Sec9 binding to Sso1.	bind
12812	2	4908	6	NULL	NULL	NULL	NULL	Vsm1	GP		bind					Sso1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_8_3114_s_75	12925750	(C) Vsm1 displaces Sec9 binding to Sso1.	bind
16304	3	4908	6	NULL	NULL	NULL	NULL	statement 2	Process		displace					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_8_3114_s_75	12925750	(C) Vsm1 displaces Sec9 binding to Sso1.	bind
14459	1	4910	5	NULL	NULL	0	NULL	Ezh2 antibodies	NULL		precipitate	NULL				Ezh2	NULL				NULL		0	NULL	NULL	NULL	gw70_development_130_18_4235_s_258	12900441	(C) Western blot analysis  of IP-bound beads and supernatant (SN) showed that the Ezh2 antibodies precipitate  Ezh2 and that Eed and HDAC1 are bound to this complex.	bind
14460	2	4910	5	NULL	NULL	0	NULL	Eed	NULL		bind	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_development_130_18_4235_s_258	12900441	(C) Western blot analysis  of IP-bound beads and supernatant (SN) showed that the Ezh2 antibodies precipitate  Ezh2 and that Eed and HDAC1 are bound to this complex.	bind
14461	3	4910	5	NULL	NULL	0	NULL	HDAC1	NULL		bind	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_development_130_18_4235_s_258	12900441	(C) Western blot analysis  of IP-bound beads and supernatant (SN) showed that the Ezh2 antibodies precipitate  Ezh2 and that Eed and HDAC1 are bound to this complex.	bind
12813	1	4910	6	NULL	NULL	NULL	NULL	Ezh2 antibodies	GP		precipitate					Ezh2	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_130_18_4235_s_258	12900441	(C) Western blot analysis  of IP-bound beads and supernatant (SN) showed that the Ezh2 antibodies precipitate  Ezh2 and that Eed and HDAC1 are bound to this complex.	bind
12814	2	4910	6	NULL	NULL	NULL	NULL	Eed	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_130_18_4235_s_258	12900441	(C) Western blot analysis  of IP-bound beads and supernatant (SN) showed that the Ezh2 antibodies precipitate  Ezh2 and that Eed and HDAC1 are bound to this complex.	bind
12815	3	4910	6	NULL	NULL	NULL	NULL	HDAC1	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_130_18_4235_s_258	12900441	(C) Western blot analysis  of IP-bound beads and supernatant (SN) showed that the Ezh2 antibodies precipitate  Ezh2 and that Eed and HDAC1 are bound to this complex.	bind
14462	2	4914	5	NULL	NULL	0	NULL	SER	NULL		does not bind	NULL				Notch	NULL				NULL		NULL	NULL	NULL	NULL	gw70_development_130_26_6411_s_310	14627724	(C) When  O-fucose is extended by Fringe, SER can not bind or activate Notch.	bind
14463	4	4914	5	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_development_130_26_6411_s_310	14627724	(C) When  O-fucose is extended by Fringe, SER can not bind or activate Notch.	bind
14464	3	4914	5	NULL	NULL	0	NULL	SER	NULL		does not activate	NULL				Notch	NULL				NULL		0	NULL	NULL	NULL	gw70_development_130_26_6411_s_310	14627724	(C) When  O-fucose is extended by Fringe, SER can not bind or activate Notch.	bind
14465	5	4914	5	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_development_130_26_6411_s_310	14627724	(C) When  O-fucose is extended by Fringe, SER can not bind or activate Notch.	bind
44578	1	4914	5	10	NULL	0	NULL	O-fucose	NULL		extended by	NULL				fringe	NULL				NULL		0	NULL	NULL	NULL	gw70_development_130_26_6411_s_310	14627724	(C) When  O-fucose is extended by Fringe, SER can not bind or activate Notch.	bind
12816	1	4914	6	NULL	NULL	NULL	NULL	o-fucose	Chemical		extended by					Fringe	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_130_26_6411_s_310	14627724	(C) When  O-fucose is extended by Fringe, SER can not bind or activate Notch.	bind
12817	2	4914	6	NULL	NULL	NULL	NULL	SER	CellComponent		does not bind					Notch	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_130_26_6411_s_310	14627724	(C) When  O-fucose is extended by Fringe, SER can not bind or activate Notch.	bind
12818	3	4914	6	NULL	NULL	NULL	NULL	SER	CellComponent		does not activate					Notch	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_130_26_6411_s_310	14627724	(C) When  O-fucose is extended by Fringe, SER can not bind or activate Notch.	bind
12819	4	4914	6	NULL	NULL	NULL	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_130_26_6411_s_310	14627724	(C) When  O-fucose is extended by Fringe, SER can not bind or activate Notch.	bind
12820	5	4914	6	NULL	NULL	NULL	NULL	statement 1	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_130_26_6411_s_310	14627724	(C) When  O-fucose is extended by Fringe, SER can not bind or activate Notch.	bind
14466	1	4915	5	NULL	NULL	0	NULL	FGF-1	NULL		bind	NULL	high affinity			FGFR2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_10_6754_s_369	10490614	(C) When heparin is added to the system where no cell surface proteoglycans are available, heparin promotes high-affinity binding of FGF-1 to FGFR2.	bind
14467	2	4915	5	NULL	NULL	0	NULL	heparin	NULL		promote	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_10_6754_s_369	10490614	(C) When heparin is added to the system where no cell surface proteoglycans are available, heparin promotes high-affinity binding of FGF-1 to FGFR2.	bind
17657	3	4915	5	NULL	NULL	0	NULL	statement 2	NULL		in the absence of	NULL				cell surface proteoglycans 	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_10_6754_s_369	10490614	(C) When heparin is added to the system where no cell surface proteoglycans are available, heparin promotes high-affinity binding of FGF-1 to FGFR2.	bind
13011	1	4915	6	NULL	NULL	NULL	NULL	FGF-1	GP		bind		high affinity			FGFR2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_6754_s_369	10490614	(C) When heparin is added to the system where no cell surface proteoglycans are available, heparin promotes high-affinity binding of FGF-1 to FGFR2.	bind
13012	2	4915	6	NULL	NULL	NULL	NULL	heparin	Chemical		promotes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_6754_s_369	10490614	(C) When heparin is added to the system where no cell surface proteoglycans are available, heparin promotes high-affinity binding of FGF-1 to FGFR2.	bind
13013	3	4915	6	NULL	NULL	NULL	NULL	statement 2	Process		occurs in absence of					cell surface proteoglycans	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_6754_s_369	10490614	(C) When heparin is added to the system where no cell surface proteoglycans are available, heparin promotes high-affinity binding of FGF-1 to FGFR2.	bind
14468	1	4916	5	NULL	NULL	0	NULL	hsc70	NULL	wild-type	bind	NULL				auxilin	NULL		J-domain		NULL		0	NULL	NULL	NULL	gw60_cellbiol_159_3_477_s_211	12427870	(C) Wild-type and mutant hsc70 bind the J-domain of auxilin.	bind
14469	2	4916	5	NULL	NULL	0	NULL	hsc70	NULL	mutant	bind	NULL				auxilin	NULL		J-domain		NULL		0	NULL	NULL	NULL	gw60_cellbiol_159_3_477_s_211	12427870	(C) Wild-type and mutant hsc70 bind the J-domain of auxilin.	bind
13014	1	4916	6	NULL	NULL	NULL	NULL	hsc70	GP	wild type	bind					auxilin	GP		J-domain		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_3_477_s_211	12427870	(C) Wild-type and mutant hsc70 bind the J-domain of auxilin.	bind
13015	2	4916	6	NULL	NULL	NULL	NULL	hsc70	GP	mutant	bind					auxilin	GP		J-domain		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_3_477_s_211	12427870	(C) Wild-type and mutant hsc70 bind the J-domain of auxilin.	bind
14470	1	4917	5	NULL	NULL	0	NULL	Sir1p	NULL	wild-type	bind	NULL					NULL			HMR	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_2_774_s_290	14701749	(C) Wild-type and mutant Sir1p binding to  HMR a was examined using ChIP assays with anti-HA.	bind
14471	2	4917	5	NULL	NULL	0	NULL	Sir1p	NULL	mutant	bind	NULL					NULL			HMR	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_2_774_s_290	14701749	(C) Wild-type and mutant Sir1p binding to  HMR a was examined using ChIP assays with anti-HA.	bind
13016	1	4917	6	NULL	NULL	NULL	NULL	Sir1p	GP	wild type	bind									HMR	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_2_774_s_290	14701749	(C) Wild-type and mutant Sir1p binding to  HMR a was examined using ChIP assays with anti-HA.	bind
13017	2	4917	6	NULL	NULL	NULL	NULL	Sir1p	GP	mutant	bind									HMR	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_2_774_s_290	14701749	(C) Wild-type and mutant Sir1p binding to  HMR a was examined using ChIP assays with anti-HA.	bind
14472	1	4918	5	NULL	NULL	0	NULL	RS	NULL		bind	NULL				chromatin	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_8_3536_s_276	15060172	(C) Wild-type p53 triggers binding of RS and RH to chromatin.	bind
14473	2	4918	5	NULL	NULL	0	NULL	p53	NULL	wild-type	triggers	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_8_3536_s_276	15060172	(C) Wild-type p53 triggers binding of RS and RH to chromatin.	bind
14474	3	4918	5	NULL	NULL	0	NULL	RH	NULL		bind	NULL				chromatin	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_8_3536_s_276	15060172	(C) Wild-type p53 triggers binding of RS and RH to chromatin.	bind
14475	4	4918	5	NULL	NULL	0	NULL	p53	NULL	wild-type	triggers	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_8_3536_s_276	15060172	(C) Wild-type p53 triggers binding of RS and RH to chromatin.	bind
13018	1	4918	6	NULL	NULL	NULL	NULL	RS	GP		bind					chromatin	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_8_3536_s_276	15060172	(C) Wild-type p53 triggers binding of RS and RH to chromatin.	bind
13019	2	4918	6	NULL	NULL	NULL	NULL	RH	GP		bind					chromatin	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_8_3536_s_276	15060172	(C) Wild-type p53 triggers binding of RS and RH to chromatin.	bind
13020	3	4918	6	NULL	NULL	NULL	NULL	p53	GP	wild type	triggers					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_8_3536_s_276	15060172	(C) Wild-type p53 triggers binding of RS and RH to chromatin.	bind
13021	4	4918	6	NULL	NULL	NULL	NULL	p53	GP	wild type	triggers					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_8_3536_s_276	15060172	(C) Wild-type p53 triggers binding of RS and RH to chromatin.	bind
14476	1	4919	5	NULL	NULL	0	NULL	DNedd4	NULL		bind	NULL		WW2		Comm	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_35_3_447_s_91	12165468	(C) WW2 and WW3 from DNedd4 can each bind Comm.	bind
14477	2	4919	5	NULL	NULL	0	NULL	DNedd4	NULL		bind	NULL		WW3		Comm	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_35_3_447_s_91	12165468	(C) WW2 and WW3 from DNedd4 can each bind Comm.	bind
13022	1	4919	6	NULL	NULL	NULL	NULL	DNedd4	GP		bind			WW2		Comm	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_35_3_447_s_91	12165468	(C) WW2 and WW3 from DNedd4 can each bind Comm.	bind
13023	2	4919	6	NULL	NULL	NULL	NULL	DNedd4	GP		bind			WW3		Comm	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_35_3_447_s_91	12165468	(C) WW2 and WW3 from DNedd4 can each bind Comm.	bind
14478	1	4920	5	NULL	NULL	0	NULL	Nkd	NULL		bind	NULL				Dsh	NULL				NULL		0	NULL	NULL	NULL	gw70_genetics_174_1_331_s_209	16849595	(C) Y2H of Nkd or Nkddelta30aa binding to Dsh or DshbPDZ.	bind
14479	2	4920	5	NULL	NULL	0	NULL	Nkd	NULL		bind	NULL		delta30aa		Dsh	NULL				NULL		0	NULL	NULL	NULL	gw70_genetics_174_1_331_s_209	16849595	(C) Y2H of Nkd or Nkddelta30aa binding to Dsh or DshbPDZ.	bind
14480	3	4920	5	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_genetics_174_1_331_s_209	16849595	(C) Y2H of Nkd or Nkddelta30aa binding to Dsh or DshbPDZ.	bind
14481	4	4920	5	NULL	NULL	0	NULL	Nkd	NULL		bind	NULL				Dshb	NULL		PDZ		NULL		0	NULL	NULL	NULL	gw70_genetics_174_1_331_s_209	16849595	(C) Y2H of Nkd or Nkddelta30aa binding to Dsh or DshbPDZ.	bind
14482	5	4920	5	NULL	NULL	0	NULL	Nkd	NULL		bind	NULL		delta30aa		Dshb	NULL		PDZ		NULL		0	NULL	NULL	NULL	gw70_genetics_174_1_331_s_209	16849595	(C) Y2H of Nkd or Nkddelta30aa binding to Dsh or DshbPDZ.	bind
14483	6	4920	5	NULL	NULL	0	NULL	statement 4	NULL		is an alternative to	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw70_genetics_174_1_331_s_209	16849595	(C) Y2H of Nkd or Nkddelta30aa binding to Dsh or DshbPDZ.	bind
13030	1	4920	6	NULL	NULL	NULL	NULL	Nkd	GP		bind					Dsh	GP				NULL		NULL	NULL	NULL	NULL	gw70_genetics_174_1_331_s_209	16849595	(C) Y2H of Nkd or Nkddelta30aa binding to Dsh or DshbPDZ.	bind
13031	2	4920	6	NULL	NULL	NULL	NULL	Nkd	GP		bind			delta30aa		Dsh	GP				NULL		NULL	NULL	NULL	NULL	gw70_genetics_174_1_331_s_209	16849595	(C) Y2H of Nkd or Nkddelta30aa binding to Dsh or DshbPDZ.	bind
13032	3	4920	6	NULL	NULL	NULL	NULL	Nkd	GP		bind					Dshb	GP		PDZ domain		NULL		NULL	NULL	NULL	NULL	gw70_genetics_174_1_331_s_209	16849595	(C) Y2H of Nkd or Nkddelta30aa binding to Dsh or DshbPDZ.	bind
13033	4	4920	6	NULL	NULL	NULL	NULL	Nkd	GP		bind			delta30aa		Dshb	GP		PDZ domain		NULL		NULL	NULL	NULL	NULL	gw70_genetics_174_1_331_s_209	16849595	(C) Y2H of Nkd or Nkddelta30aa binding to Dsh or DshbPDZ.	bind
54592	5	4920	6	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_genetics_174_1_331_s_209	16849595	(C) Y2H of Nkd or Nkddelta30aa binding to Dsh or DshbPDZ.	bind
54593	6	4920	6	NULL	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_genetics_174_1_331_s_209	16849595	(C) Y2H of Nkd or Nkddelta30aa binding to Dsh or DshbPDZ.	bind
14484	1	4921	5	NULL	NULL	0	NULL	LFY	NULL		bind	NULL				AP3	NULL			site I	NULL		0	NULL	NULL	NULL	gw60_development_129_9_2079_s_126	11959818	(C) Yeast one-hybrid assays demonstrate that LFY binds to  AP3 site I.	bind
13036	1	4921	6	NULL	NULL	NULL	NULL	LFY	GP		bind					AP3	GP			site I 	NULL		NULL	NULL	NULL	NULL	gw60_development_129_9_2079_s_126	11959818	(C) Yeast one-hybrid assays demonstrate that LFY binds to  AP3 site I.	bind
14485	1	4923	5	NULL	NULL	0	NULL	Smad3	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_13_4494_s_178	12808092	(C) YY1  inhibits DNA binding of Smad3 and Smad4.	bind
14486	2	4923	5	NULL	NULL	0	NULL	Smad4	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_13_4494_s_178	12808092	(C) YY1  inhibits DNA binding of Smad3 and Smad4.	bind
14487	3	4923	5	NULL	NULL	0	NULL	YY1	NULL		inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_13_4494_s_178	12808092	(C) YY1  inhibits DNA binding of Smad3 and Smad4.	bind
14488	4	4923	5	NULL	NULL	0	NULL	YY1	NULL		inhibit	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_13_4494_s_178	12808092	(C) YY1  inhibits DNA binding of Smad3 and Smad4.	bind
13038	1	4923	6	NULL	NULL	NULL	NULL	Smad3	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_13_4494_s_178	12808092	(C) YY1  inhibits DNA binding of Smad3 and Smad4.	bind
13039	2	4923	6	NULL	NULL	NULL	NULL	Smad4	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_13_4494_s_178	12808092	(C) YY1  inhibits DNA binding of Smad3 and Smad4.	bind
13041	3	4923	6	NULL	NULL	NULL	NULL	YY1	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_13_4494_s_178	12808092	(C) YY1  inhibits DNA binding of Smad3 and Smad4.	bind
13042	4	4923	6	NULL	NULL	NULL	NULL	YY1	GP		inhibits					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_13_4494_s_178	12808092	(C) YY1  inhibits DNA binding of Smad3 and Smad4.	bind
14489	2	4925	5	10	NULL	0	NULL	GTP S			bind					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_neuron_38_2_291_s_179	12718862	(C) [35]GTP S binding to HEK-293 cell membranes expressing D3R/Go  was determined after stimulation with dopamine.	bind
14490	3	4925	5	10	NULL	0	NULL	statement 1	NULL		occurs after stimulation with	NULL				dopamine	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuron_38_2_291_s_179	12718862	(C) [35]GTP S binding to HEK-293 cell membranes expressing D3R/Go  was determined after stimulation with dopamine.	bind
44579	1	4925	5	10	NULL	0	NULL	HEK-293 cell membranes	NULL		express	NULL				D3R/Go	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_38_2_291_s_179	12718862	(C) [35]GTP S binding to HEK-293 cell membranes expressing D3R/Go  was determined after stimulation with dopamine.	bind
13044	1	4925	6	NULL	NULL	NULL	NULL	HEK-293 cell membranes	CellComponent		express					D3R/Go	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_38_2_291_s_179	12718862	(C) [35]GTP S binding to HEK-293 cell membranes expressing D3R/Go  was determined after stimulation with dopamine.	bind
13046	2	4925	6	NULL	NULL	NULL	NULL	GTP S	Chemical		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_38_2_291_s_179	12718862	(C) [35]GTP S binding to HEK-293 cell membranes expressing D3R/Go  was determined after stimulation with dopamine.	bind
13049	3	4925	6	NULL	NULL	NULL	NULL	dopamine	Chemical		stimulates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_38_2_291_s_179	12718862	(C) [35]GTP S binding to HEK-293 cell membranes expressing D3R/Go  was determined after stimulation with dopamine.	bind
14491	1	4926	5	10	NULL	0	NULL	GTP			bind					Xl Sept2					NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_21_1858_s_34	12419187	(C) [3]GTP binding of  Xl Sept2 and  cc-Sep2, as determined by a filter binding assay.	bind
14492	2	4926	5	10	NULL	0	NULL	GTP			bind					cc-Sep2					NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_21_1858_s_34	12419187	(C) [3]GTP binding of  Xl Sept2 and  cc-Sep2, as determined by a filter binding assay.	bind
13051	1	4926	6	NULL	NULL	NULL	NULL	GTP	Chemical		bind					Xl Sept2	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_21_1858_s_34	12419187	(C) [3]GTP binding of  Xl Sept2 and  cc-Sep2, as determined by a filter binding assay.	bind
13052	2	4926	6	NULL	NULL	NULL	NULL	GTP	Chemical		bind					cc-Sep2	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_21_1858_s_34	12419187	(C) [3]GTP binding of  Xl Sept2 and  cc-Sep2, as determined by a filter binding assay.	bind
14493	1	4927	5	NULL	NULL	0	NULL	Siah-1	NULL		bind	NULL				pAPC	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_molcell_7_5_927_s_47	11389840	(C), (D), and (E) show in vitro and in vivo binding of Siah-1 to pAPC.	bind
14494	2	4927	5	NULL	NULL	0	NULL	Siah-1	NULL		bind	NULL				pAPC	NULL				NULL	in vivo	0	NULL	NULL	NULL	gw60_molcell_7_5_927_s_47	11389840	(C), (D), and (E) show in vitro and in vivo binding of Siah-1 to pAPC.	bind
13055	1	4927	6	NULL	NULL	NULL	NULL	Siah-1	GP		bind					pAPC	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcell_7_5_927_s_47	11389840	(C), (D), and (E) show in vitro and in vivo binding of Siah-1 to pAPC.	bind
13056	2	4927	6	NULL	NULL	NULL	NULL	Siah-1	GP		bind					pAPC	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcell_7_5_927_s_47	11389840	(C), (D), and (E) show in vitro and in vivo binding of Siah-1 to pAPC.	bind
14495	1	4929	5	NULL	NULL	0	NULL	TFIIIA	NULL		bind	NULL				DNA	NULL	nucleosomal			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_6_2167_s_85	10688663	(C, D, and E) Removal of the core histone tails or the H2A-H2B dimer facilitates TFIIIA binding to nucleosomal DNA.	bind
14496	2	4929	5	NULL	NULL	0	NULL	core histone tails	NULL	removal of	facilitate	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_6_2167_s_85	10688663	(C, D, and E) Removal of the core histone tails or the H2A-H2B dimer facilitates TFIIIA binding to nucleosomal DNA.	bind
14497	3	4929	5	NULL	NULL	0	NULL	H2A-H2B dimer	NULL	removal of	facilitate	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_6_2167_s_85	10688663	(C, D, and E) Removal of the core histone tails or the H2A-H2B dimer facilitates TFIIIA binding to nucleosomal DNA.	bind
14498	4	4929	5	NULL	NULL	0	NULL	statement 2	NULL		is an alternative to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_6_2167_s_85	10688663	(C, D, and E) Removal of the core histone tails or the H2A-H2B dimer facilitates TFIIIA binding to nucleosomal DNA.	bind
13057	1	4929	6	NULL	NULL	NULL	NULL	TFIIIA	GP		bind					nucleosomal DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2167_s_85	10688663	(C, D, and E) Removal of the core histone tails or the H2A-H2B dimer facilitates TFIIIA binding to nucleosomal DNA.	bind
13058	2	4929	6	NULL	NULL	NULL	NULL	core histone tails		removal of	facilitate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2167_s_85	10688663	(C, D, and E) Removal of the core histone tails or the H2A-H2B dimer facilitates TFIIIA binding to nucleosomal DNA.	bind
13059	3	4929	6	NULL	NULL	NULL	NULL	H2A-H2B dimer	GP	removal of	facilitate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2167_s_85	10688663	(C, D, and E) Removal of the core histone tails or the H2A-H2B dimer facilitates TFIIIA binding to nucleosomal DNA.	bind
13060	4	4929	6	NULL	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2167_s_85	10688663	(C, D, and E) Removal of the core histone tails or the H2A-H2B dimer facilitates TFIIIA binding to nucleosomal DNA.	bind
14499	1	4930	5	NULL	NULL	0	NULL	Par3L isoforms	NULL		bind	NULL	differentially			Par6	NULL				NULL		0	NULL	NULL	NULL	gw60_gene_294_1_99_s_202	12234671	(C,D) Par3L isoforms show differential binding to Par6.	bind
13061	1	4930	6	NULL	NULL	NULL	NULL	Par3L isoforms	GP		bind		differentially			Par6	GP				NULL		NULL	NULL	NULL	NULL	gw60_gene_294_1_99_s_202	12234671	(C,D) Par3L isoforms show differential binding to Par6.	bind
14500	1	4931	5	NULL	NULL	0	NULL	GFR 1-Fc receptor bodies	NULL		bind	NULL	directly			GDNF ligands	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_6_1291_s_171	9883723	(C-E) Direct binding of GFR 1-Fc (C), GFR 2-Fc (D), and GFR 3-Fc (E) receptor bodies to the GDNF ligands.	bind
14501	2	4931	5	NULL	NULL	0	NULL	GFR 2-Fc receptor bodies	NULL		bind	NULL	directly			GDNF ligands	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_21_6_1291_s_171	9883723	(C-E) Direct binding of GFR 1-Fc (C), GFR 2-Fc (D), and GFR 3-Fc (E) receptor bodies to the GDNF ligands.	bind
14502	3	4931	5	NULL	NULL	0	NULL	GFR 3-Fc receptor bodies	NULL		bind	NULL	directly			GDNF ligands	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_21_6_1291_s_171	9883723	(C-E) Direct binding of GFR 1-Fc (C), GFR 2-Fc (D), and GFR 3-Fc (E) receptor bodies to the GDNF ligands.	bind
13062	1	4931	6	NULL	NULL	NULL	NULL	GFR 1-Fc receptor body	GP		bind		directly			GDNF ligands	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_6_1291_s_171	9883723	(C-E) Direct binding of GFR 1-Fc (C), GFR 2-Fc (D), and GFR 3-Fc (E) receptor bodies to the GDNF ligands.	bind
13063	2	4931	6	NULL	NULL	NULL	NULL	GFR 2-Fc receptor body	GP		bind		directly			GDNF ligands	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_6_1291_s_171	9883723	(C-E) Direct binding of GFR 1-Fc (C), GFR 2-Fc (D), and GFR 3-Fc (E) receptor bodies to the GDNF ligands.	bind
13064	3	4931	6	NULL	NULL	NULL	NULL	GFR 3-Fc receptor body	GP		bind		directly			GDNF ligands	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_6_1291_s_171	9883723	(C-E) Direct binding of GFR 1-Fc (C), GFR 2-Fc (D), and GFR 3-Fc (E) receptor bodies to the GDNF ligands.	bind
14503	1	4932	5	10	NULL	0	NULL	SKP1			bind					CUL1					NULL	HeLa cells	NULL	NULL	NULL	NULL	gw60_molcell_10_6_1519_s_175	12504026	(C-E) Silencing of CAND1 in HeLa cells caused increased binding of SKP1 and SKP2 to CUL1 and downregulation of SKP2.	bind
14504	2	4932	5	NULL	NULL	0	NULL	CAND1	NULL	silencing of	increase	NULL				statement 1	NULL				NULL	in HeLa cells	NULL	NULL	NULL	NULL	gw60_molcell_10_6_1519_s_175	12504026	(C-E) Silencing of CAND1 in HeLa cells caused increased binding of SKP1 and SKP2 to CUL1 and downregulation of SKP2.	bind
14505	3	4932	5	10	NULL	0	NULL	SKP2			bind					CUL1					NULL	HeLa cells	NULL	NULL	NULL	NULL	gw60_molcell_10_6_1519_s_175	12504026	(C-E) Silencing of CAND1 in HeLa cells caused increased binding of SKP1 and SKP2 to CUL1 and downregulation of SKP2.	bind
14506	4	4932	5	NULL	NULL	0	NULL	CAND1	NULL	silencing of	increase	NULL				statement 3	NULL				NULL	in HeLa cells	NULL	NULL	NULL	NULL	gw60_molcell_10_6_1519_s_175	12504026	(C-E) Silencing of CAND1 in HeLa cells caused increased binding of SKP1 and SKP2 to CUL1 and downregulation of SKP2.	bind
14507	5	4932	5	NULL	NULL	0	NULL	CAND1	NULL	silencing of	downregulates	NULL				Skp2	NULL				NULL	in HeLa cells	NULL	NULL	NULL	NULL	gw60_molcell_10_6_1519_s_175	12504026	(C-E) Silencing of CAND1 in HeLa cells caused increased binding of SKP1 and SKP2 to CUL1 and downregulation of SKP2.	bind
13065	1	4932	6	NULL	NULL	NULL	NULL	SKP1	GP		bind					CUL1	GP				NULL	HeLa cells	NULL	NULL	NULL	NULL	gw60_molcell_10_6_1519_s_175	12504026	(C-E) Silencing of CAND1 in HeLa cells caused increased binding of SKP1 and SKP2 to CUL1 and downregulation of SKP2.	bind
13066	2	4932	6	NULL	NULL	NULL	NULL	SKP2	GP		bind					CUL1	GP				NULL	HeLa cells	NULL	NULL	NULL	NULL	gw60_molcell_10_6_1519_s_175	12504026	(C-E) Silencing of CAND1 in HeLa cells caused increased binding of SKP1 and SKP2 to CUL1 and downregulation of SKP2.	bind
13067	3	4932	6	NULL	NULL	NULL	NULL	CAND1	GP	silencing of	increases					statement 1	Process				NULL	HeLa cells	NULL	NULL	NULL	NULL	gw60_molcell_10_6_1519_s_175	12504026	(C-E) Silencing of CAND1 in HeLa cells caused increased binding of SKP1 and SKP2 to CUL1 and downregulation of SKP2.	bind
13068	4	4932	6	NULL	NULL	NULL	NULL	CAND1	GP	silencing of	increases					statement 2	Process				NULL	HeLa cells	NULL	NULL	NULL	NULL	gw60_molcell_10_6_1519_s_175	12504026	(C-E) Silencing of CAND1 in HeLa cells caused increased binding of SKP1 and SKP2 to CUL1 and downregulation of SKP2.	bind
13069	5	4932	6	NULL	NULL	NULL	NULL	CAND1	GP	silencing of	downregulates					SKP2	GP				NULL	HeLa cells	NULL	NULL	NULL	NULL	gw60_molcell_10_6_1519_s_175	12504026	(C-E) Silencing of CAND1 in HeLa cells caused increased binding of SKP1 and SKP2 to CUL1 and downregulation of SKP2.	bind
14508	1	4935	5	NULL	NULL	0	NULL	(CAG)(n)-hairpin DNA	NULL		bind	NULL				Msh2-Msh3	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_nat-struct-mol-biol_12_8_16025128_s_1	16025128	(CAG)(n)-hairpin DNA binds to Msh2-Msh3 and changes properties of mismatch recognition..	bind
14509	2	4935	5	NULL	NULL	0	NULL	(CAG)(n)-hairpin DNA	NULL		change	NULL				mismatch recognition	NULL	properties of			NULL		0	NULL	NULL	NULL	abs-batch0620-0649_nat-struct-mol-biol_12_8_16025128_s_1	16025128	(CAG)(n)-hairpin DNA binds to Msh2-Msh3 and changes properties of mismatch recognition..	bind
13071	1	4935	6	NULL	NULL	NULL	NULL	(CAG)(n)-hairpin DNA	NucleicAcid		bind					Msh2-Msh3	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_nat-struct-mol-biol_12_8_16025128_s_1	16025128	(CAG)(n)-hairpin DNA binds to Msh2-Msh3 and changes properties of mismatch recognition..	bind
13072	2	4935	6	NULL	NULL	NULL	NULL	statement 1	Process		changes					mismatch recognition	Process	properties of 			NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_nat-struct-mol-biol_12_8_16025128_s_1	16025128	(CAG)(n)-hairpin DNA binds to Msh2-Msh3 and changes properties of mismatch recognition..	bind
14510	1	4938	5	NULL	NULL	0	NULL	Crk-associated substrate	NULL		bind	NULL		SH3 domain		FAK	NULL		proline-rich region		NULL		NULL	NULL	NULL	NULL	gw60_febslett_498_1_26_s_13	11389892	(Crk-associated substrate) binds the proline-rich region of FAK through an SH3 domain.	bind
13073	1	4938	6	NULL	NULL	NULL	NULL	Crk-associated substrate	GP		bind			SH3 domain		FAK	GP		proline-rich region		NULL		NULL	NULL	NULL	NULL	gw60_febslett_498_1_26_s_13	11389892	(Crk-associated substrate) binds the proline-rich region of FAK through an SH3 domain.	bind
14511	1	4939	5	NULL	NULL	0	NULL	Csk-associated substrate	NULL		bind	NULL		SH2 domain		Src kinase	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_10_8837_s_374	12496276	(Csk-associated substrate) binds Src kinase through its SH2 and SH3 domains ( ).	bind
14512	2	4939	5	NULL	NULL	0	NULL	Csk-associated substrate	NULL		bind	NULL		SH3 domain		Src kinase	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_10_8837_s_374	12496276	(Csk-associated substrate) binds Src kinase through its SH2 and SH3 domains ( ).	bind
13074	1	4939	6	NULL	NULL	NULL	NULL	Csk-associated substrate	GP		bind			SH2 domain		Src kinase	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_10_8837_s_374	12496276	(Csk-associated substrate) binds Src kinase through its SH2 and SH3 domains ( ).	bind
13075	2	4939	6	NULL	NULL	NULL	NULL	Csk-associated substrate	GP		bind			SH3 domain		Src kinase	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_10_8837_s_374	12496276	(Csk-associated substrate) binds Src kinase through its SH2 and SH3 domains ( ).	bind
14513	1	4941	5	10	NULL	0	NULL				bind				(CT)n regions	GAGA factor					NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_nucleic-acids-res_31_10_12736297_s_3	12736297	(CT)n  regions are known to bind GAGA factor, a dominant enhancer of PEV thought  to play a role in generating an accessible chromatin structure.	bind
14514	2	4941	5	10	NULL	0	NULL	GAGA factor			is a type of					PEV		dominant		  enhancer 	NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_nucleic-acids-res_31_10_12736297_s_3	12736297	(CT)n  regions are known to bind GAGA factor, a dominant enhancer of PEV thought  to play a role in generating an accessible chromatin structure.	bind
54594	3	4941	5	10	NULL	0	NULL	statement 1			plays a role in					chromatin structure		generating;; accessible			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_nucleic-acids-res_31_10_12736297_s_3	12736297	(CT)n  regions are known to bind GAGA factor, a dominant enhancer of PEV thought  to play a role in generating an accessible chromatin structure.	bind
13076	1	4941	6	NULL	NULL	NULL	NULL	GAGA factor	GP		is a type of					PEV	GP	dominant		enhancer	NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_nucleic-acids-res_31_10_12736297_s_3	12736297	(CT)n  regions are known to bind GAGA factor, a dominant enhancer of PEV thought  to play a role in generating an accessible chromatin structure.	bind
13077	2	4941	6	NULL	NULL	NULL	NULL	statement 1	Process		plays a role in					chromatin	OrganismPart	generating an;; accessible;;  structure of			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_nucleic-acids-res_31_10_12736297_s_3	12736297	(CT)n  regions are known to bind GAGA factor, a dominant enhancer of PEV thought  to play a role in generating an accessible chromatin structure.	bind
13078	3	4941	6	NULL	NULL	NULL	NULL				bind				(CT)n regions	GAGA factor	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_nucleic-acids-res_31_10_12736297_s_3	12736297	(CT)n  regions are known to bind GAGA factor, a dominant enhancer of PEV thought  to play a role in generating an accessible chromatin structure.	bind
14517	1	4943	5	NULL	NULL	0	NULL	Krox-20	NULL		activate	NULL				periaxin protein	NULL	expression of			NULL	in Swiss 3T3 cells	0	NULL	NULL	NULL	gw70_cellbiol_164_3_385_s_91	14757751	(D - G) Krox-20 activates periaxin and P0 myelin protein expression in Swiss 3T3 cells.	bind
14518	2	4943	5	NULL	NULL	0	NULL	Krox-20	NULL		activate	NULL				P0 myelin protein	NULL	expression of			NULL	in Swiss 3T3 cells	0	NULL	NULL	NULL	gw70_cellbiol_164_3_385_s_91	14757751	(D - G) Krox-20 activates periaxin and P0 myelin protein expression in Swiss 3T3 cells.	bind
13144	1	4943	6	NULL	NULL	NULL	NULL	Krox-20	GP		activates					periaxin protein	GP	expression of			NULL	Swiss 3T3 cells	NULL	NULL	NULL	NULL	gw70_cellbiol_164_3_385_s_91	14757751	(D - G) Krox-20 activates periaxin and P0 myelin protein expression in Swiss 3T3 cells.	bind
13145	2	4943	6	NULL	NULL	NULL	NULL	Krox-20	GP		activates					P0 myelin protein	GP	expression of			NULL	Swiss 3T3 cells	NULL	NULL	NULL	NULL	gw70_cellbiol_164_3_385_s_91	14757751	(D - G) Krox-20 activates periaxin and P0 myelin protein expression in Swiss 3T3 cells.	bind
14519	1	4944	5	NULL	NULL	0	NULL	Pol I	NULL		bind	NULL				35S rDNA	NULL			promoter	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_32_19_5851_s_242	15520468	(D and E)  In vitro binding of Pol I to the 35S rDNA promoter.	bind
13146	1	4944	6	NULL	NULL	NULL	NULL	Pol I	GP		bind					35S rDNA	NucleicAcid			promoter	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_32_19_5851_s_242	15520468	(D and E)  In vitro binding of Pol I to the 35S rDNA promoter.	bind
14520	1	4945	5	NULL	NULL	0	NULL		NULL		bind	NULL		GST-ARD		Tiam1	NULL	recombinant	C1199		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_cellbiol_150_1_177_s_279	10893266	(D and E) Binding analysis between GST-ARD and the recombinant C1199 Tiam1 in vitro.	bind
13147	1	4945	6	NULL	NULL	NULL	NULL				bind			GST-ARD		Tiam1	GP	recombinant	C1199		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_cellbiol_150_1_177_s_279	10893266	(D and E) Binding analysis between GST-ARD and the recombinant C1199 Tiam1 in vitro.	bind
14521	2	4946	5	NULL	NULL	0	NULL	Cdc31p	NULL		bind	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_162_7_1211_s_164	14504268	(d and e) Cdc31p binding to Sfi1p fusions containing 1 - 3  repeats.	bind
44580	1	4946	5	10	NULL	0	NULL	Sfi1p fusions	NULL		contain	NULL					NULL		1-3 repeats		NULL		0	NULL	NULL	NULL	gw70_cellbiol_162_7_1211_s_164	14504268	(d and e) Cdc31p binding to Sfi1p fusions containing 1 - 3  repeats.	bind
13148	1	4946	6	NULL	NULL	NULL	NULL	Sfi1p fusions	GP		contain								1-3 repeats		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_162_7_1211_s_164	14504268	(d and e) Cdc31p binding to Sfi1p fusions containing 1 - 3  repeats.	bind
13149	2	4946	6	NULL	NULL	NULL	NULL	Cdc31p	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_162_7_1211_s_164	14504268	(d and e) Cdc31p binding to Sfi1p fusions containing 1 - 3  repeats.	bind
14522	2	4947	5	10	NULL	0	NULL	statement 1			dephosphorylate					TbetaRI					NULL	in vivo	NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_291_s_142	14718519	(d and e) In in vivo  dephosphorylation assay, dominant-negative SARA with a mutation in the PP1c-binding  domain (F728A) inhibits the dephosphorylation of TbetaRI by Smad7-recruited PP1 complex.	bind
14523	3	4947	5	10	NULL	0	NULL	SARA		dominant-negative mutant 	inhibit			PP1c-binding domain;;F728A		statement 1					NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_291_s_142	14718519	(d and e) In in vivo  dephosphorylation assay, dominant-negative SARA with a mutation in the PP1c-binding  domain (F728A) inhibits the dephosphorylation of TbetaRI by Smad7-recruited PP1 complex.	bind
54595	1	4947	5	10	NULL	0	NULL	Smad7			recruit					PP1 complex					NULL		0	NULL	NULL	NULL	gw70_cellbiol_164_2_291_s_142	14718519	(d and e) In in vivo  dephosphorylation assay, dominant-negative SARA with a mutation in the PP1c-binding  domain (F728A) inhibits the dephosphorylation of TbetaRI by Smad7-recruited PP1 complex.	bind
13322	2	4947	6	NULL	NULL	NULL	NULL	statement 1	Process		dephosphorylates					TbetaRI	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_291_s_142	14718519	(d and e) In in vivo  dephosphorylation assay, dominant-negative SARA with a mutation in the PP1c-binding  domain (F728A) inhibits the dephosphorylation of TbetaRI by Smad7-recruited PP1 complex.	bind
13323	3	4947	6	NULL	NULL	NULL	NULL	SARA	GP	dominant-negative mutant	inhibits			PP1c-binding domain;;F728A		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_291_s_142	14718519	(d and e) In in vivo  dephosphorylation assay, dominant-negative SARA with a mutation in the PP1c-binding  domain (F728A) inhibits the dephosphorylation of TbetaRI by Smad7-recruited PP1 complex.	bind
54596	1	4947	6	NULL	NULL	NULL	NULL	Smad7	GP		recruits					PP1 complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_291_s_142	14718519	(d and e) In in vivo  dephosphorylation assay, dominant-negative SARA with a mutation in the PP1c-binding  domain (F728A) inhibits the dephosphorylation of TbetaRI by Smad7-recruited PP1 complex.	bind
14524	1	4948	5	NULL	NULL	0	NULL	MEF2C	NULL		bind	NULL				p300	NULL				NULL	in cardiocytes	0	NULL	NULL	NULL	gw60_molcellbiol_20_23_8643_s_174	11073966	(D and E) MEF2C binds p300 in cardiocytes.	bind
13150	1	4948	6	NULL	NULL	NULL	NULL	MEF2C	GP		bind					p300	GP				NULL	cardiocytes	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_23_8643_s_174	11073966	(D and E) MEF2C binds p300 in cardiocytes.	bind
14525	1	4950	5	NULL	NULL	0	NULL	myc-Snf5p	NULL		bind	NULL				SNZ1	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8829_s_246	14612422	(D and H) The strains described for panels A and E that harbor the  SNF5-myc allele were subjected to ChIP analysis to measure binding of myc-Snf5p to  SNZ1.	bind
13151	1	4950	6	NULL	NULL	NULL	NULL	myc-Snf5p	GP		bind					SNZ1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8829_s_246	14612422	(D and H) The strains described for panels A and E that harbor the  SNF5-myc allele were subjected to ChIP analysis to measure binding of myc-Snf5p to  SNZ1.	bind
14526	1	4951	5	NULL	NULL	0	NULL	Dynamin	NULL		bind	NULL				Amphiphysin	NULL		SH3 domain		NULL		0	NULL	NULL	NULL	gw60_development_128_24_5005_s_90	11748137	(D)  Drosophila Amphiphysin does not interact with  Drosophila Dynamin: western analysis and Coomassie staining of Dynamin binding to the SH3 domain of Amphiphysin.	bind
14527	2	4951	5	NULL	NULL	0	NULL	Amphiphysin	NULL	Drosophila	does not interact with	NULL				Dynamin	NULL	Drosophila			NULL		0	NULL	NULL	NULL	gw60_development_128_24_5005_s_90	11748137	(D)  Drosophila Amphiphysin does not interact with  Drosophila Dynamin: western analysis and Coomassie staining of Dynamin binding to the SH3 domain of Amphiphysin.	bind
13152	1	4951	6	NULL	NULL	NULL	NULL	Amphiphysin	GP	Drosophila	does not interact					Dynamin	GP	Drosophila			NULL		NULL	NULL	NULL	NULL	gw60_development_128_24_5005_s_90	11748137	(D)  Drosophila Amphiphysin does not interact with  Drosophila Dynamin: western analysis and Coomassie staining of Dynamin binding to the SH3 domain of Amphiphysin.	bind
13153	2	4951	6	NULL	NULL	NULL	NULL	Dynamin	GP		bind					Amphiphysin	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_development_128_24_5005_s_90	11748137	(D)  Drosophila Amphiphysin does not interact with  Drosophila Dynamin: western analysis and Coomassie staining of Dynamin binding to the SH3 domain of Amphiphysin.	bind
14528	1	4953	5	10	NULL	0	NULL	Nkx2-5			bind					Hop				Nkx2.5 binding site in proximal promoter	NULL		NULL	NULL	NULL	NULL	gw60_cell_110_6_713_s_112	12297045	(D) (left) EMSA revealing that Nkx2-5 can bind to a Nkx2.5 binding site (NKE-WT) present in the proximal Hop promoter, while it can not bind a mutant Nkx2.5 binding site (mut).	bind
14529	2	4953	5	10	NULL	0	NULL	Nkx2-5			does not bind					Hop		mutant		Nkx2.5 binding site	NULL		NULL	NULL	NULL	NULL	gw60_cell_110_6_713_s_112	12297045	(D) (left) EMSA revealing that Nkx2-5 can bind to a Nkx2.5 binding site (NKE-WT) present in the proximal Hop promoter, while it can not bind a mutant Nkx2.5 binding site (mut).	bind
54597	3	4953	5	10	NULL	0	NULL	NKE-WT			is					wild type Nkx2.5 binding site					NULL		0	NULL	NULL	NULL	gw60_cell_110_6_713_s_112	12297045	(D) (left) EMSA revealing that Nkx2-5 can bind to a Nkx2.5 binding site (NKE-WT) present in the proximal Hop promoter, while it can not bind a mutant Nkx2.5 binding site (mut).	bind
13154	1	4953	6	NULL	NULL	NULL	NULL	Nkx2-5	GP		bind					Hop	GP			NKE-WT of proximal promoter	NULL		NULL	NULL	NULL	NULL	gw60_cell_110_6_713_s_112	12297045	(D) (left) EMSA revealing that Nkx2-5 can bind to a Nkx2.5 binding site (NKE-WT) present in the proximal Hop promoter, while it can not bind a mutant Nkx2.5 binding site (mut).	bind
13155	2	4953	6	NULL	NULL	NULL	NULL	NKE-WT	GP		is							wild type		 Nkx2.5 binding site 	NULL		NULL	NULL	NULL	NULL	gw60_cell_110_6_713_s_112	12297045	(D) (left) EMSA revealing that Nkx2-5 can bind to a Nkx2.5 binding site (NKE-WT) present in the proximal Hop promoter, while it can not bind a mutant Nkx2.5 binding site (mut).	bind
13156	3	4953	6	NULL	NULL	NULL	NULL	Nkx2-5	GP		does not bind					Hop	GP	mutant		Nkx2.5 binding site	NULL		NULL	NULL	NULL	NULL	gw60_cell_110_6_713_s_112	12297045	(D) (left) EMSA revealing that Nkx2-5 can bind to a Nkx2.5 binding site (NKE-WT) present in the proximal Hop promoter, while it can not bind a mutant Nkx2.5 binding site (mut).	bind
14530	1	4954	5	NULL	NULL	0	NULL	GST-RB	NULL		does not bind	NULL	directly			p53	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_3_2_181_s_183	10078201	(D) (right panel) shows that GST-RB does not bind to p53 directly, and it can only coprecipitate with p53 in the presence of MDM2.	bind
14531	2	4954	5	10	NULL	0	NULL	GST-RB			bind					p53					NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_2_181_s_183	10078201	(D) (right panel) shows that GST-RB does not bind to p53 directly, and it can only coprecipitate with p53 in the presence of MDM2.	bind
14532	3	4954	5	NULL	NULL	0	NULL	statement 2	NULL		in the presence of	NULL	only			MDM2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_3_2_181_s_183	10078201	(D) (right panel) shows that GST-RB does not bind to p53 directly, and it can only coprecipitate with p53 in the presence of MDM2.	bind
13158	1	4954	6	NULL	NULL	NULL	NULL	GST-RB	GP		does not bind		directly			p53	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_2_181_s_183	10078201	(D) (right panel) shows that GST-RB does not bind to p53 directly, and it can only coprecipitate with p53 in the presence of MDM2.	bind
13159	2	4954	6	NULL	NULL	NULL	NULL	GST-RB	GP		bind					p53	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_2_181_s_183	10078201	(D) (right panel) shows that GST-RB does not bind to p53 directly, and it can only coprecipitate with p53 in the presence of MDM2.	bind
13160	3	4954	6	NULL	NULL	NULL	NULL	statement 2	Process		occurs in presence of		only			MDM2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_2_181_s_183	10078201	(D) (right panel) shows that GST-RB does not bind to p53 directly, and it can only coprecipitate with p53 in the presence of MDM2.	bind
14533	1	4955	5	NULL	NULL	0	NULL	Vav	NULL		bind	NULL		SH2 domain		SLP-76	NULL				NULL		0	NULL	NULL	NULL	gw60_immunity_6_2_155_s_134	9047237	(D) (Top panel) Peptides corresponding to the first pYESP motifs can compete for Vav SH2 domain binding to SLP-76.	bind
14534	2	4955	5	NULL	NULL	0	NULL	Peptides	NULL		bind	NULL		pYESP motifs		SLP-76	NULL				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_2_155_s_134	9047237	(D) (Top panel) Peptides corresponding to the first pYESP motifs can compete for Vav SH2 domain binding to SLP-76.	bind
14535	3	4955	5	NULL	NULL	0	NULL	statement 2	NULL		compete with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_immunity_6_2_155_s_134	9047237	(D) (Top panel) Peptides corresponding to the first pYESP motifs can compete for Vav SH2 domain binding to SLP-76.	bind
13161	1	4955	6	NULL	NULL	NULL	NULL	Vav	GP		bind			SH2 domain		SLP-76	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_2_155_s_134	9047237	(D) (Top panel) Peptides corresponding to the first pYESP motifs can compete for Vav SH2 domain binding to SLP-76.	bind
13162	2	4955	6	NULL	NULL	NULL	NULL	peptide			bind			pYESP motifs		SLP-76	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_2_155_s_134	9047237	(D) (Top panel) Peptides corresponding to the first pYESP motifs can compete for Vav SH2 domain binding to SLP-76.	bind
13163	3	4955	6	NULL	NULL	NULL	NULL	statement 1	Process		competes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_2_155_s_134	9047237	(D) (Top panel) Peptides corresponding to the first pYESP motifs can compete for Vav SH2 domain binding to SLP-76.	bind
14536	1	4957	5	NULL	NULL	0	NULL	Sp1	NULL		bind	NULL				p21WAF1/CIP1	NULL			GC-rich region of the promoter	NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_7_979_s_36	15051732	(d) 1 ng/ml of TGFbeta1 enhanced  the binding of Sp1 to a GC-rich region in the p21WAF1/CIP1 promoter as determined by chromatin immunoprecipitation.	bind
14537	2	4957	5	NULL	NULL	0	NULL	TGFbeta1	NULL		enhances	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_164_7_979_s_36	15051732	(d) 1 ng/ml of TGFbeta1 enhanced  the binding of Sp1 to a GC-rich region in the p21WAF1/CIP1 promoter as determined by chromatin immunoprecipitation.	bind
13164	1	4957	6	NULL	NULL	NULL	NULL	Sp1	GP		bind					p21WAF1/CIP1	GP			GC-rich region of the promoter	NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_7_979_s_36	15051732	(d) 1 ng/ml of TGFbeta1 enhanced  the binding of Sp1 to a GC-rich region in the p21WAF1/CIP1 promoter as determined by chromatin immunoprecipitation.	bind
13165	2	4957	6	NULL	NULL	NULL	NULL	TGFbeta1	GP		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_7_979_s_36	15051732	(d) 1 ng/ml of TGFbeta1 enhanced  the binding of Sp1 to a GC-rich region in the p21WAF1/CIP1 promoter as determined by chromatin immunoprecipitation.	bind
14538	1	4958	5	NULL	NULL	0	NULL	24 hpf embryo	NULL		express	NULL	ectopically			Nkx6 (fly gene) RNA	NULL	ectopic 			NULL		NULL	NULL	NULL	NULL	gw70_development_131_21_5221_s_286	15456722	(D) 24 hpf embryo ectopically expressing  Nkx6 (fly gene) RNA generates ectopic PMNs (compare with  Fig. 7D).	bind
17658	2	4958	5	NULL	NULL	0	NULL	statement 1	NULL		generates	NULL				PMN	NULL	ectopic			NULL		0	NULL	NULL	NULL	gw70_development_131_21_5221_s_286	15456722	(D) 24 hpf embryo ectopically expressing  Nkx6 (fly gene) RNA generates ectopic PMNs (compare with  Fig. 7D).	bind
13166	1	4958	6	NULL	NULL	NULL	NULL	24 hpf embryo	Organism		express		ectopically			Nkx6 (fly gene) RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_development_131_21_5221_s_286	15456722	(D) 24 hpf embryo ectopically expressing  Nkx6 (fly gene) RNA generates ectopic PMNs (compare with  Fig. 7D).	bind
13167	2	4958	6	NULL	NULL	NULL	NULL	statement 1	Process		generates					PMN	Cell	ectopic			NULL		NULL	NULL	NULL	NULL	gw70_development_131_21_5221_s_286	15456722	(D) 24 hpf embryo ectopically expressing  Nkx6 (fly gene) RNA generates ectopic PMNs (compare with  Fig. 7D).	bind
14539	1	4959	5	NULL	NULL	0	NULL	prohibitin	NULL	35S-labeled	bind	NULL				GST-Suv39H	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw70_molcellbiol_26_11_4161_s_142	16705168	(D) 35S-labeled prohibitin binds to GST-Suv39H in vitro.	bind
13168	1	4959	6	NULL	NULL	NULL	NULL	prohibitin	GP	35S-labeled	bind					GST-Suv39H	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4161_s_142	16705168	(D) 35S-labeled prohibitin binds to GST-Suv39H in vitro.	bind
14540	3	4960	5	NULL	NULL	0	NULL	statement 1	NULL		occur along with	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_140	10330164	(D) A chimeric protein containing the amino terminus of TFIIB and the cyclin homology domain of cyclin E does not bind to p300.	bind
44581	1	4960	5	10	NULL	0	NULL	chimeric protein	NULL		contains	NULL				TFIIB	NULL		 amino terminus		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_140	10330164	(D) A chimeric protein containing the amino terminus of TFIIB and the cyclin homology domain of cyclin E does not bind to p300.	bind
44582	2	4960	5	10	NULL	0	NULL	chimeric protein	NULL		contain	NULL				cyclin E	NULL		cyclin homology domain		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_140	10330164	(D) A chimeric protein containing the amino terminus of TFIIB and the cyclin homology domain of cyclin E does not bind to p300.	bind
44583	4	4960	5	10	NULL	0	NULL	statement 3	NULL		does not bind	NULL				p300	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_140	10330164	(D) A chimeric protein containing the amino terminus of TFIIB and the cyclin homology domain of cyclin E does not bind to p300.	bind
13169	3	4960	6	NULL	NULL	NULL	NULL	statement 1	Process		occur along with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_140	10330164	(D) A chimeric protein containing the amino terminus of TFIIB and the cyclin homology domain of cyclin E does not bind to p300.	bind
41943	4	4960	6	NULL	NULL	NULL	NULL	statement 3	Process		does not bind					p300	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_140	10330164	(D) A chimeric protein containing the amino terminus of TFIIB and the cyclin homology domain of cyclin E does not bind to p300.	bind
54598	1	4960	6	NULL	NULL	NULL	NULL	chimeric protein	GP		contains					TFIIB	GP		amino terminus of		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_140	10330164	(D) A chimeric protein containing the amino terminus of TFIIB and the cyclin homology domain of cyclin E does not bind to p300.	bind
54600	2	4960	6	NULL	NULL	NULL	NULL	chimeric protein	GP		contains					cyclin E	GP		cyclin homology domain		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_140	10330164	(D) A chimeric protein containing the amino terminus of TFIIB and the cyclin homology domain of cyclin E does not bind to p300.	bind
14541	2	4961	5	NULL	NULL	0	NULL	VASP	NULL	His-tagged	bind	NULL		EVH1 domain		Ni	NULL				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_18_1617_s_21	12372256	(D) A Coomassie-stained gel showing that the His-tagged EVH1 domain of VASP, from a soluble  E.  coli extract (sol), binds to the nickel resin (Ni) and the positive control ActA peptide FPPPP, but not to the negative control ActA peptide APPPP or residues 451-461 of WIP (peptide F).	bind
14542	3	4961	5	NULL	NULL	0	NULL	Ni	NULL		is	NULL				nickel resin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_18_1617_s_21	12372256	(D) A Coomassie-stained gel showing that the His-tagged EVH1 domain of VASP, from a soluble  E.  coli extract (sol), binds to the nickel resin (Ni) and the positive control ActA peptide FPPPP, but not to the negative control ActA peptide APPPP or residues 451-461 of WIP (peptide F).	bind
14543	4	4961	5	NULL	NULL	0	NULL	VASP	NULL	His-tagged 	bind	NULL		EVH1 domain		ActA peptide FPPPP	NULL	positive control			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_18_1617_s_21	12372256	(D) A Coomassie-stained gel showing that the His-tagged EVH1 domain of VASP, from a soluble  E.  coli extract (sol), binds to the nickel resin (Ni) and the positive control ActA peptide FPPPP, but not to the negative control ActA peptide APPPP or residues 451-461 of WIP (peptide F).	bind
14544	5	4961	5	NULL	NULL	0	NULL	VASP	NULL	His-tagged	does not bind	NULL		EVH1 domain		ActA peptide APPPP	NULL	negative control			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_18_1617_s_21	12372256	(D) A Coomassie-stained gel showing that the His-tagged EVH1 domain of VASP, from a soluble  E.  coli extract (sol), binds to the nickel resin (Ni) and the positive control ActA peptide FPPPP, but not to the negative control ActA peptide APPPP or residues 451-461 of WIP (peptide F).	bind
14545	6	4961	5	NULL	NULL	0	NULL	VASP	NULL	His-tagged	does not bind	NULL		EVH1 domain		WIP	NULL		residues 451-461		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_18_1617_s_21	12372256	(D) A Coomassie-stained gel showing that the His-tagged EVH1 domain of VASP, from a soluble  E.  coli extract (sol), binds to the nickel resin (Ni) and the positive control ActA peptide FPPPP, but not to the negative control ActA peptide APPPP or residues 451-461 of WIP (peptide F).	bind
44584	1	4961	5	10	NULL	0	NULL	VASP	NULL		is derived from	NULL		EVH1 domain		soluble E.coli extract	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_12_18_1617_s_21	12372256	(D) A Coomassie-stained gel showing that the His-tagged EVH1 domain of VASP, from a soluble  E.  coli extract (sol), binds to the nickel resin (Ni) and the positive control ActA peptide FPPPP, but not to the negative control ActA peptide APPPP or residues 451-461 of WIP (peptide F).	bind
13325	1	4961	6	NULL	NULL	NULL	NULL	VASP	GP		bind			EVH1 domain		ActA peptide FPPPP	GP	positive control			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_18_1617_s_21	12372256	(D) A Coomassie-stained gel showing that the His-tagged EVH1 domain of VASP, from a soluble  E.  coli extract (sol), binds to the nickel resin (Ni) and the positive control ActA peptide FPPPP, but not to the negative control ActA peptide APPPP or residues 451-461 of WIP (peptide F).	bind
13326	2	4961	6	NULL	NULL	NULL	NULL	VASP	GP		does not bind			EVH1 domain		ActA peptide FPPPP	GP	negative control			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_18_1617_s_21	12372256	(D) A Coomassie-stained gel showing that the His-tagged EVH1 domain of VASP, from a soluble  E.  coli extract (sol), binds to the nickel resin (Ni) and the positive control ActA peptide FPPPP, but not to the negative control ActA peptide APPPP or residues 451-461 of WIP (peptide F).	bind
13327	3	4961	6	NULL	NULL	NULL	NULL	VASP	GP		does not bind			EVH1 domain		WIP	GP		residues 451-461		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_18_1617_s_21	12372256	(D) A Coomassie-stained gel showing that the His-tagged EVH1 domain of VASP, from a soluble  E.  coli extract (sol), binds to the nickel resin (Ni) and the positive control ActA peptide FPPPP, but not to the negative control ActA peptide APPPP or residues 451-461 of WIP (peptide F).	bind
13329	4	4961	6	NULL	NULL	NULL	NULL	VASP	GP		is derived from			EVH1 domain		E.coli extract	OrganismPart	soluble			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_18_1617_s_21	12372256	(D) A Coomassie-stained gel showing that the His-tagged EVH1 domain of VASP, from a soluble  E.  coli extract (sol), binds to the nickel resin (Ni) and the positive control ActA peptide FPPPP, but not to the negative control ActA peptide APPPP or residues 451-461 of WIP (peptide F).	bind
17347	5	4961	6	NULL	NULL	NULL	NULL	Ni	Chemical		is					Nickel resin					NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_18_1617_s_21	12372256	(D) A Coomassie-stained gel showing that the His-tagged EVH1 domain of VASP, from a soluble  E.  coli extract (sol), binds to the nickel resin (Ni) and the positive control ActA peptide FPPPP, but not to the negative control ActA peptide APPPP or residues 451-461 of WIP (peptide F).	bind
17348	6	4961	6	NULL	NULL	NULL	NULL	VASP	GP		bind			EVH1 domain		Ni	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_18_1617_s_21	12372256	(D) A Coomassie-stained gel showing that the His-tagged EVH1 domain of VASP, from a soluble  E.  coli extract (sol), binds to the nickel resin (Ni) and the positive control ActA peptide FPPPP, but not to the negative control ActA peptide APPPP or residues 451-461 of WIP (peptide F).	bind
14546	1	4962	5	NULL	NULL	0	NULL	Rb	NULL		mediate	NULL				E2F	NULL	repression of;; activity of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7487_s_195	9819434	(D) A dominant-acting form of Ras can reverse Rb-mediated repression of E2F activity.	bind
14547	2	4962	5	NULL	NULL	0	NULL	Ras	NULL	dominant-acting form of	reverse	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_12_7487_s_195	9819434	(D) A dominant-acting form of Ras can reverse Rb-mediated repression of E2F activity.	bind
13171	1	4962	6	NULL	NULL	NULL	NULL	Rb	GP		mediates					E2F	GP	repression of;; activity of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7487_s_195	9819434	(D) A dominant-acting form of Ras can reverse Rb-mediated repression of E2F activity.	bind
13172	2	4962	6	NULL	NULL	NULL	NULL	Ras	GP	a dominant acting form of	reverse					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7487_s_195	9819434	(D) A dominant-acting form of Ras can reverse Rb-mediated repression of E2F activity.	bind
14548	1	4963	5	NULL	NULL	0	NULL	CRM1	NULL		bind	NULL	specifically	493-600		XAP1	NULL				NULL		0	NULL	NULL	NULL	gw60_chembiol_7_5_345_s_147	10801471	(d) A fragment of 108 amino acids (CRM1[493-600]) comprising amino acids known to affect LMB sensitivity in  S. pombe binds specifically to XAP1.	bind
17659	2	4963	5	10	NULL	0	NULL	CRM1			affect			amino acid 493-600		LMB 		sensitivity of			NULL	S. pombe	NULL	NULL	NULL	NULL	gw60_chembiol_7_5_345_s_147	10801471	(d) A fragment of 108 amino acids (CRM1[493-600]) comprising amino acids known to affect LMB sensitivity in  S. pombe binds specifically to XAP1.	bind
13330	1	4963	6	NULL	NULL	NULL	NULL	CRM1	GP		bind		specifically	amino acid 493-600		XAP1	GP				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_7_5_345_s_147	10801471	(d) A fragment of 108 amino acids (CRM1[493-600]) comprising amino acids known to affect LMB sensitivity in  S. pombe binds specifically to XAP1.	bind
13331	2	4963	6	NULL	NULL	NULL	NULL	CRM1	GP		affect			amino acid 493-600		LMB	GP	sensitivity of			NULL	S. pombe	NULL	NULL	NULL	NULL	gw60_chembiol_7_5_345_s_147	10801471	(d) A fragment of 108 amino acids (CRM1[493-600]) comprising amino acids known to affect LMB sensitivity in  S. pombe binds specifically to XAP1.	bind
14549	1	4964	5	NULL	NULL	0	NULL	SHP2-SH2-GST	NULL		bind	NULL				CAT	NULL	biotinylated;; wt			NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_148	15556604	(D) A pre-incubation of SHP2-SH2-GST with  wt CAT, but not wife Y280F, inhibits a further binding of SHP2-SH2-GST to biotinylated  wt CAT.	bind
14550	4	4964	5	NULL	NULL	0	NULL	statement 2	NULL		inhibit	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_148	15556604	(D) A pre-incubation of SHP2-SH2-GST with  wt CAT, but not wife Y280F, inhibits a further binding of SHP2-SH2-GST to biotinylated  wt CAT.	bind
14551	5	4964	5	NULL	NULL	0	NULL	statement 3	NULL		does not inhibit	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_148	15556604	(D) A pre-incubation of SHP2-SH2-GST with  wt CAT, but not wife Y280F, inhibits a further binding of SHP2-SH2-GST to biotinylated  wt CAT.	bind
44585	2	4964	5	10	NULL	0	NULL	SHP2-SH2-GST	NULL		pre-incubated with	NULL				CAT	NULL	wt			NULL		0	NULL	NULL	NULL	gw70_febslett_577_3_327_s_148	15556604	(D) A pre-incubation of SHP2-SH2-GST with  wt CAT, but not wife Y280F, inhibits a further binding of SHP2-SH2-GST to biotinylated  wt CAT.	bind
44586	3	4964	5	10	NULL	0	NULL	SHP2-SH2-GST	NULL		pre-incubated with	NULL				wife	NULL		Y280F		NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_148	15556604	(D) A pre-incubation of SHP2-SH2-GST with  wt CAT, but not wife Y280F, inhibits a further binding of SHP2-SH2-GST to biotinylated  wt CAT.	bind
13174	1	4964	6	NULL	NULL	NULL	NULL	SHP2-SH2-GST 			bind					CAT	GP	biotinylated;; wild type			NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_148	15556604	(D) A pre-incubation of SHP2-SH2-GST with  wt CAT, but not wife Y280F, inhibits a further binding of SHP2-SH2-GST to biotinylated  wt CAT.	bind
13175	2	4964	6	NULL	NULL	NULL	NULL	SHP2-SH2-GST 			pre incubated with					CAT	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_148	15556604	(D) A pre-incubation of SHP2-SH2-GST with  wt CAT, but not wife Y280F, inhibits a further binding of SHP2-SH2-GST to biotinylated  wt CAT.	bind
13176	3	4964	6	NULL	NULL	NULL	NULL	statement 2	Process		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_148	15556604	(D) A pre-incubation of SHP2-SH2-GST with  wt CAT, but not wife Y280F, inhibits a further binding of SHP2-SH2-GST to biotinylated  wt CAT.	bind
13177	4	4964	6	NULL	NULL	NULL	NULL	SHP2-SH2-GST			pre incubated with					wife	GP		Y280F		NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_148	15556604	(D) A pre-incubation of SHP2-SH2-GST with  wt CAT, but not wife Y280F, inhibits a further binding of SHP2-SH2-GST to biotinylated  wt CAT.	bind
13178	5	4964	6	NULL	NULL	NULL	NULL	statement 4	Process		does not inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_febslett_577_3_327_s_148	15556604	(D) A pre-incubation of SHP2-SH2-GST with  wt CAT, but not wife Y280F, inhibits a further binding of SHP2-SH2-GST to biotinylated  wt CAT.	bind
14552	1	4966	5	NULL	NULL	0	NULL	PR	NULL	full-length	bind	NULL				Src	NULL		SH3 domain		NULL		0	NULL	NULL	NULL	gw60_molcell_8_2_269_s_48	11545730	(D) A synthetic peptide containing the PR proline-rich motif inhibits interaction of full-length PR with the SH3 domain of Src. PR-B binding to GST-Src (U-SH3-SH2 domains) by a pull-down assay was performed as in (C), except in the presence and absence of varying concentrations of a synthetic peptide (200- to 3000-fold molar excess over PR-B) containing either the wild-type PR proline-rich motif (WT) or a mutant motif (Mut).	bind
14553	2	4966	5	NULL	NULL	0	NULL	peptide	NULL	synthetic	inhibit	NULL		PR proline-rich motif		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_8_2_269_s_48	11545730	(D) A synthetic peptide containing the PR proline-rich motif inhibits interaction of full-length PR with the SH3 domain of Src. PR-B binding to GST-Src (U-SH3-SH2 domains) by a pull-down assay was performed as in (C), except in the presence and absence of varying concentrations of a synthetic peptide (200- to 3000-fold molar excess over PR-B) containing either the wild-type PR proline-rich motif (WT) or a mutant motif (Mut).	bind
14554	3	4966	5	NULL	NULL	0	NULL	PR-B	NULL		bind	NULL				GST-Src	NULL		U-SH3-SH2 domains		NULL		0	NULL	NULL	NULL	gw60_molcell_8_2_269_s_48	11545730	(D) A synthetic peptide containing the PR proline-rich motif inhibits interaction of full-length PR with the SH3 domain of Src. PR-B binding to GST-Src (U-SH3-SH2 domains) by a pull-down assay was performed as in (C), except in the presence and absence of varying concentrations of a synthetic peptide (200- to 3000-fold molar excess over PR-B) containing either the wild-type PR proline-rich motif (WT) or a mutant motif (Mut).	bind
13179	1	4966	6	NULL	NULL	NULL	NULL	PR	GP	full length	interacts with					Src	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_2_269_s_48	11545730	(D) A synthetic peptide containing the PR proline-rich motif inhibits interaction of full-length PR with the SH3 domain of Src. PR-B binding to GST-Src (U-SH3-SH2 domains) by a pull-down assay was performed as in (C), except in the presence and absence of varying concentrations of a synthetic peptide (200- to 3000-fold molar excess over PR-B) containing either the wild-type PR proline-rich motif (WT) or a mutant motif (Mut).	bind
13180	2	4966	6	NULL	NULL	NULL	NULL	PR-B	GP		bind					GST-Src	GP		U-SH3-SH2 domains		NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_2_269_s_48	11545730	(D) A synthetic peptide containing the PR proline-rich motif inhibits interaction of full-length PR with the SH3 domain of Src. PR-B binding to GST-Src (U-SH3-SH2 domains) by a pull-down assay was performed as in (C), except in the presence and absence of varying concentrations of a synthetic peptide (200- to 3000-fold molar excess over PR-B) containing either the wild-type PR proline-rich motif (WT) or a mutant motif (Mut).	bind
13181	3	4966	6	NULL	NULL	NULL	NULL	peptide		synthetic	contains					PR	GP		proline-rich motifs		NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_2_269_s_48	11545730	(D) A synthetic peptide containing the PR proline-rich motif inhibits interaction of full-length PR with the SH3 domain of Src. PR-B binding to GST-Src (U-SH3-SH2 domains) by a pull-down assay was performed as in (C), except in the presence and absence of varying concentrations of a synthetic peptide (200- to 3000-fold molar excess over PR-B) containing either the wild-type PR proline-rich motif (WT) or a mutant motif (Mut).	bind
13182	4	4966	6	NULL	NULL	NULL	NULL	statement 3	Process		inhibits					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_2_269_s_48	11545730	(D) A synthetic peptide containing the PR proline-rich motif inhibits interaction of full-length PR with the SH3 domain of Src. PR-B binding to GST-Src (U-SH3-SH2 domains) by a pull-down assay was performed as in (C), except in the presence and absence of varying concentrations of a synthetic peptide (200- to 3000-fold molar excess over PR-B) containing either the wild-type PR proline-rich motif (WT) or a mutant motif (Mut).	bind
14555	1	4967	5	NULL	NULL	0	NULL	UNC-115	NULL		bind	NULL		VHD		actin	NULL				NULL		0	NULL	NULL	NULL	gw70_development_130_4_693_s_269	12506000	(D) A western blot showing that the  UNC-115 VHD bound to actin.	bind
13183	1	4967	6	NULL	NULL	NULL	NULL	UNC-115	GP		bind			VHD		actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_130_4_693_s_269	12506000	(D) A western blot showing that the  UNC-115 VHD bound to actin.	bind
14556	1	4969	5	NULL	NULL	0	NULL	Mgamma proteins	NULL		bind	NULL				N-box probe	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_7_4600_s_110	10373509	(D) Addition of a fivefold molar excess of unlabeled B1 oligonucleotide has a greater effect on binding of the Mgamma and Mbeta proteins (approximately 500 ng of soluble pGex fusion protein) to the N-box probe than addition of a fivefold excess molar excess of unlabeled N-box oligonucleotide.	bind
14557	2	4969	5	NULL	NULL	0	NULL	Mbeta proteins	NULL		bind	NULL				N-box probe	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_7_4600_s_110	10373509	(D) Addition of a fivefold molar excess of unlabeled B1 oligonucleotide has a greater effect on binding of the Mgamma and Mbeta proteins (approximately 500 ng of soluble pGex fusion protein) to the N-box probe than addition of a fivefold excess molar excess of unlabeled N-box oligonucleotide.	bind
13184	1	4969	6	NULL	NULL	NULL	NULL	Mgamma proteins	GP		bind					N-box probe					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4600_s_110	10373509	(D) Addition of a fivefold molar excess of unlabeled B1 oligonucleotide has a greater effect on binding of the Mgamma and Mbeta proteins (approximately 500 ng of soluble pGex fusion protein) to the N-box probe than addition of a fivefold excess molar excess of unlabeled N-box oligonucleotide.	bind
13185	2	4969	6	NULL	NULL	NULL	NULL	Mbeta proteins	GP		bind					N-box probe					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4600_s_110	10373509	(D) Addition of a fivefold molar excess of unlabeled B1 oligonucleotide has a greater effect on binding of the Mgamma and Mbeta proteins (approximately 500 ng of soluble pGex fusion protein) to the N-box probe than addition of a fivefold excess molar excess of unlabeled N-box oligonucleotide.	bind
14558	1	4970	5	10	NULL	0	NULL	Claspin	NULL		bind	NULL				chromatin	NULL				NULL	RPA-depleted extracts	NULL	NULL	NULL	NULL	gw60_molcell_11_2_329_s_164	12620222	(D) Addition of rhRPA to RPA-depleted extracts restores normally regulated binding of Claspin and Pol   to chromatin.	bind
14559	2	4970	5	NULL	NULL	0	NULL	Pol 	NULL		bind	NULL				chromatin	NULL				NULL	RPA-depleted extracts	NULL	NULL	NULL	NULL	gw60_molcell_11_2_329_s_164	12620222	(D) Addition of rhRPA to RPA-depleted extracts restores normally regulated binding of Claspin and Pol   to chromatin.	bind
14560	3	4970	5	10	NULL	0	NULL	rhRPA	NULL	addition of	restores	NULL				statement 1	NULL	normally regulated			NULL	RPA-depleted extracts	NULL	NULL	NULL	NULL	gw60_molcell_11_2_329_s_164	12620222	(D) Addition of rhRPA to RPA-depleted extracts restores normally regulated binding of Claspin and Pol   to chromatin.	bind
14561	4	4970	5	10	NULL	0	NULL	rhRPA	NULL	addition of	restores	NULL				statement 2	NULL	normally regulated			NULL	RPA-depleted extracts	NULL	NULL	NULL	NULL	gw60_molcell_11_2_329_s_164	12620222	(D) Addition of rhRPA to RPA-depleted extracts restores normally regulated binding of Claspin and Pol   to chromatin.	bind
13187	1	4970	6	NULL	NULL	NULL	NULL	Claspin	GP		bind					chromatin	OrganismPart				NULL	RPA-depleted extracts	NULL	NULL	NULL	NULL	gw60_molcell_11_2_329_s_164	12620222	(D) Addition of rhRPA to RPA-depleted extracts restores normally regulated binding of Claspin and Pol   to chromatin.	bind
13188	2	4970	6	NULL	NULL	NULL	NULL	Pol	GP		bind					chromatin	OrganismPart				NULL	RPA-depleted extracts	NULL	NULL	NULL	NULL	gw60_molcell_11_2_329_s_164	12620222	(D) Addition of rhRPA to RPA-depleted extracts restores normally regulated binding of Claspin and Pol   to chromatin.	bind
13189	3	4970	6	NULL	NULL	NULL	NULL	rhRPA	GP	addition of	restores					statement 1	Process	normally regulated			NULL	RPA-depleted extracts	NULL	NULL	NULL	NULL	gw60_molcell_11_2_329_s_164	12620222	(D) Addition of rhRPA to RPA-depleted extracts restores normally regulated binding of Claspin and Pol   to chromatin.	bind
13190	4	4970	6	NULL	NULL	NULL	NULL	rhRPA	GP	addition of	restores					statement 2	Process	normally regulated			NULL	RPA-depleted extracts	NULL	NULL	NULL	NULL	gw60_molcell_11_2_329_s_164	12620222	(D) Addition of rhRPA to RPA-depleted extracts restores normally regulated binding of Claspin and Pol   to chromatin.	bind
14562	1	4971	5	NULL	NULL	0	NULL	GST-SF-1 protein	NULL	recombinant	bind	NULL				AMH	NULL			SF-1-BS in promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_11_6653_s_188	9774680	(D) Affinity binding of GST-SF-1 recombinant protein to the SF-1-binding site (SF-1-BS) in the AMH promoter.	bind
14563	2	4971	5	NULL	NULL	0	NULL	SF-1-BS	NULL		is	NULL				SF-1-binding site	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_11_6653_s_188	9774680	(D) Affinity binding of GST-SF-1 recombinant protein to the SF-1-binding site (SF-1-BS) in the AMH promoter.	bind
13191	1	4971	6	NULL	NULL	NULL	NULL	GST-SF-1 protein	GP	recombinant	bind					AMH	GP			SF-1-BS of promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_11_6653_s_188	9774680	(D) Affinity binding of GST-SF-1 recombinant protein to the SF-1-binding site (SF-1-BS) in the AMH promoter.	bind
13192	2	4971	6	NULL	NULL	NULL	NULL	SF-1-BS			is					SF-1-binding site					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_11_6653_s_188	9774680	(D) Affinity binding of GST-SF-1 recombinant protein to the SF-1-binding site (SF-1-BS) in the AMH promoter.	bind
14564	1	4972	5	NULL	NULL	0	NULL	importin-alpha receptors	NULL		bind	NULL				SV40	NULL		NLS		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_11_4159_s_238	10805757	(D) All the importin-alpha receptors tested can bind to the SV40 NLS.	bind
13193	1	4972	6	NULL	NULL	NULL	NULL	importin-alpha receptors	GP		bind					SV40	GP		NLS		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_11_4159_s_238	10805757	(D) All the importin-alpha receptors tested can bind to the SV40 NLS.	bind
14565	1	4973	5	10	NULL	0	NULL	TSP1	NULL		mediate	NULL		alpha4beta1 integrin binding regions		CD4+T cells	NULL	adhesion of ;;activated			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_3_509_s_53	11980922	(D) alpha4beta1 integrin binding regions of TSP1 and TSP2 mediate adhesion of activated CD4+T cells.	bind
14566	2	4973	5	10	NULL	0	NULL	TSP2	NULL		mediate	NULL		alpha4beta1 integrin binding regions		CD4+T cells	NULL	adhesion of ;;activated			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_3_509_s_53	11980922	(D) alpha4beta1 integrin binding regions of TSP1 and TSP2 mediate adhesion of activated CD4+T cells.	bind
13194	1	4973	6	NULL	NULL	NULL	NULL	TSP1	GP		mediate			alpha4beta1 integrin binding regions		CD4+T cells	Cell	adhesion of;; activated			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_3_509_s_53	11980922	(D) alpha4beta1 integrin binding regions of TSP1 and TSP2 mediate adhesion of activated CD4+T cells.	bind
13195	2	4973	6	NULL	NULL	NULL	NULL	TSP2	GP		mediate			alpha4beta1 integrin binding regions		CD4+T cells	Cell	adhesion of;; activated			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_3_509_s_53	11980922	(D) alpha4beta1 integrin binding regions of TSP1 and TSP2 mediate adhesion of activated CD4+T cells.	bind
14567	1	4974	5	NULL	NULL	0	NULL	RPA	NULL		bind	NULL				GST-Stuho	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_152_5_985_s_226	11238454	(D) Amount of RPA bound to GST-Stuho.	bind
13196	1	4974	6	NULL	NULL	NULL	NULL	RPA	GP		bind					GST-Stuho	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_985_s_226	11238454	(D) Amount of RPA bound to GST-Stuho.	bind
14569	1	4976	5	NULL	NULL	0	NULL	Axin	NULL		bind	NULL				LRP6deltaEGF-FKBP	NULL				NULL	in 293 cells	0	NULL	NULL	NULL	gw70_development_131_20_5103_s_180	15459103	(D) AP20187 increases the binding of Axin to LRP6deltaEGF-FKBP during beta-catenin stabilization in 293 cells.	bind
14570	2	4976	5	NULL	NULL	0	NULL	statement 1	NULL		occurs during	NULL				beta-catenin 	NULL	stabilization of			NULL	in 293 cells	0	NULL	NULL	NULL	gw70_development_131_20_5103_s_180	15459103	(D) AP20187 increases the binding of Axin to LRP6deltaEGF-FKBP during beta-catenin stabilization in 293 cells.	bind
14571	3	4976	5	NULL	NULL	0	NULL	AP20187	NULL		increase	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_development_131_20_5103_s_180	15459103	(D) AP20187 increases the binding of Axin to LRP6deltaEGF-FKBP during beta-catenin stabilization in 293 cells.	bind
13197	1	4976	6	NULL	NULL	NULL	NULL	Axin	GP		bind					LRP6deltaEGF-FKBP	GP				NULL	293 cells	NULL	NULL	NULL	NULL	gw70_development_131_20_5103_s_180	15459103	(D) AP20187 increases the binding of Axin to LRP6deltaEGF-FKBP during beta-catenin stabilization in 293 cells.	bind
13198	2	4976	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs during					beta-catenin	GP	stabilization of 			NULL		NULL	NULL	NULL	NULL	gw70_development_131_20_5103_s_180	15459103	(D) AP20187 increases the binding of Axin to LRP6deltaEGF-FKBP during beta-catenin stabilization in 293 cells.	bind
13199	3	4976	6	NULL	NULL	NULL	NULL	AP20187			increases					statement 1	Process				NULL	293 cells	NULL	NULL	NULL	NULL	gw70_development_131_20_5103_s_180	15459103	(D) AP20187 increases the binding of Axin to LRP6deltaEGF-FKBP during beta-catenin stabilization in 293 cells.	bind
14572	1	4980	5	NULL	NULL	0	NULL	SRP	NULL		bind	NULL				bt-SR 	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_162_4_575_s_173	12913112	(D) Association and dissociation curves for binding of SRP to bt-SR in the presence of buffer E adjusted to (a) 25 muM GTP, (b) 25 muM GDP, or (c) 25 muM Gpp(NH)p.	bind
13200	1	4980	6	NULL	NULL	NULL	NULL	SRP	GP		bind					bt-SR	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_162_4_575_s_173	12913112	(D) Association and dissociation curves for binding of SRP to bt-SR in the presence of buffer E adjusted to (a) 25 muM GTP, (b) 25 muM GDP, or (c) 25 muM Gpp(NH)p.	bind
14574	1	4982	5	NULL	NULL	0	NULL	B7h-Ig	NULL		bind	NULL				T cells	NULL	activated			NULL		0	NULL	NULL	NULL	gw60_immunity_11_4_423_s_121	10549624	(D) B7h-Ig binds to activated T cells.	bind
13201	1	4982	6	NULL	NULL	NULL	NULL	B7h-Ig	GP		bind					T cells	Cell	activated			NULL		NULL	NULL	NULL	NULL	gw60_immunity_11_4_423_s_121	10549624	(D) B7h-Ig binds to activated T cells.	bind
14653	1	4984	5	NULL	NULL	0	NULL	Chk2	NULL	bacterially produced	bind	NULL		FHA domain		HA-Chk2	NULL		SCD		NULL	293 cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4419_s_77	12024051	(D) Bacterially produced FHA domain of Chk2 binds to SCD in HA-Chk2 and its mutants expressed in 293 cells after gamma irradiation.	bind
14654	2	4984	5	NULL	NULL	0	NULL	gamma irradiation	NULL		is required for	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_12_4419_s_77	12024051	(D) Bacterially produced FHA domain of Chk2 binds to SCD in HA-Chk2 and its mutants expressed in 293 cells after gamma irradiation.	bind
14655	3	4984	5	NULL	NULL	0	NULL	Chk2	NULL	bacterially produced	bind	NULL		FHA domain		HA-Chk2	NULL	mutants expressed	SCD		NULL	293 cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4419_s_77	12024051	(D) Bacterially produced FHA domain of Chk2 binds to SCD in HA-Chk2 and its mutants expressed in 293 cells after gamma irradiation.	bind
14656	4	4984	5	NULL	NULL	0	NULL	gamma irradiation	NULL		is required for	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_12_4419_s_77	12024051	(D) Bacterially produced FHA domain of Chk2 binds to SCD in HA-Chk2 and its mutants expressed in 293 cells after gamma irradiation.	bind
13202	1	4984	6	NULL	NULL	NULL	NULL	Chk2	GP	Bacterially produced	bind			FHA domain		HA-Chk2 	GP		SCD		NULL	293 cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4419_s_77	12024051	(D) Bacterially produced FHA domain of Chk2 binds to SCD in HA-Chk2 and its mutants expressed in 293 cells after gamma irradiation.	bind
13203	2	4984	6	NULL	NULL	NULL	NULL	Chk2	GP	Bacterially produced	bind			FHA domain		HA-Chk2 	GP	mutant	SCD		NULL	293T cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4419_s_77	12024051	(D) Bacterially produced FHA domain of Chk2 binds to SCD in HA-Chk2 and its mutants expressed in 293 cells after gamma irradiation.	bind
17349	3	4984	6	NULL	NULL	NULL	NULL	gamma radiation			is required for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4419_s_77	12024051	(D) Bacterially produced FHA domain of Chk2 binds to SCD in HA-Chk2 and its mutants expressed in 293 cells after gamma irradiation.	bind
17350	4	4984	6	NULL	NULL	NULL	NULL	gamma radiation			is required for					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4419_s_77	12024051	(D) Bacterially produced FHA domain of Chk2 binds to SCD in HA-Chk2 and its mutants expressed in 293 cells after gamma irradiation.	bind
14657	1	4985	5	NULL	NULL	0	NULL	BAF complex	NULL		does not bind	NULL				CSF1	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_cell_106_3_309_s_136	11509180	(D) BAF complex and NFI/CTF are not  bound to the CSF1 promoter when the  NFI/CTF site is mutated.	bind
14658	2	4985	5	NULL	NULL	0	NULL	statement 1	NULL		occurs on	NULL					NULL	mutation		NFI/CTF site	NULL		0	NULL	NULL	NULL	gw60_cell_106_3_309_s_136	11509180	(D) BAF complex and NFI/CTF are not  bound to the CSF1 promoter when the  NFI/CTF site is mutated.	bind
14659	3	4985	5	NULL	NULL	0	NULL	NFI/CTF	NULL		does not bind	NULL				CSF1	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_cell_106_3_309_s_136	11509180	(D) BAF complex and NFI/CTF are not  bound to the CSF1 promoter when the  NFI/CTF site is mutated.	bind
14660	4	4985	5	NULL	NULL	0	NULL	statement 3	NULL		occurs on	NULL					NULL	mutation		NFI/CTF site	NULL		0	NULL	NULL	NULL	gw60_cell_106_3_309_s_136	11509180	(D) BAF complex and NFI/CTF are not  bound to the CSF1 promoter when the  NFI/CTF site is mutated.	bind
13332	1	4985	6	NULL	NULL	NULL	NULL	BAF complex	GP		does not bind					CSF1 	GP	mutant		NFI/CTF site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_cell_106_3_309_s_136	11509180	(D) BAF complex and NFI/CTF are not  bound to the CSF1 promoter when the  NFI/CTF site is mutated.	bind
13333	2	4985	6	NULL	NULL	NULL	NULL	NFI/CTF	GP		does not bind					CSF1	GP	mutant		NFI/CTF site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_cell_106_3_309_s_136	11509180	(D) BAF complex and NFI/CTF are not  bound to the CSF1 promoter when the  NFI/CTF site is mutated.	bind
14661	1	4986	5	NULL	NULL	0	NULL	Che-1	NULL		bind	NULL				Tau	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellneurosci_24_4_1038_s_60	14697667	(D) Binding  of Che-1 by Tau affinity chromatography.	bind
13204	1	4986	6	NULL	NULL	NULL	NULL	Che-1	GP		bind					Tau	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_24_4_1038_s_60	14697667	(D) Binding  of Che-1 by Tau affinity chromatography.	bind
14662	1	4987	5	NULL	NULL	0	NULL	dATF-2	NULL		bind	NULL					NULL			CRE	NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_6_2934_s_166	15788564	(D) Binding  of dATF-2 to the CRE.	bind
13205	1	4987	6	NULL	NULL	NULL	NULL	dATF-2	GP		bind									CRE	NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_6_2934_s_166	15788564	(D) Binding  of dATF-2 to the CRE.	bind
14663	1	4991	5	NULL	NULL	0	NULL	ER	NULL		bind	NULL				SMRT	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_312_3_656_s_67	14680815	(D) Binding between ER  and SMRT was examined  using the mammalian two-hybrid system.	bind
13206	1	4991	6	NULL	NULL	NULL	NULL	ER	CellComponent		bind					SMRT	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_312_3_656_s_67	14680815	(D) Binding between ER  and SMRT was examined  using the mammalian two-hybrid system.	bind
14664	1	4992	5	NULL	NULL	0	NULL	NuMA	NULL		translated from	NULL		amino acid sequence 1831-2102		NuMA3/TOPO	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_1_29_s_226	10189366	(D) Binding of 4.1R/GST to NuMA amino acid sequence 1831-2102 translated from NuMA3/TOPO.	bind
14665	2	4992	5	NULL	NULL	0	NULL	4.1R/GST	NULL		bind	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_1_29_s_226	10189366	(D) Binding of 4.1R/GST to NuMA amino acid sequence 1831-2102 translated from NuMA3/TOPO.	bind
13207	1	4992	6	NULL	NULL	NULL	NULL	4.1R/GST	GP		bind					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_1_29_s_226	10189366	(D) Binding of 4.1R/GST to NuMA amino acid sequence 1831-2102 translated from NuMA3/TOPO.	bind
13208	2	4992	6	NULL	NULL	NULL	NULL	NuMA	GP		translated from			amino acid sequence 1831-2102		NuMA3/TOPO	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_1_29_s_226	10189366	(D) Binding of 4.1R/GST to NuMA amino acid sequence 1831-2102 translated from NuMA3/TOPO.	bind
14666	1	4993	5	NULL	NULL	0	NULL	espin constructs	NULL	6X His-tagged	bind	NULL				GST-profilin IIa	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_163_5_1045_s_175	14657236	(D) Binding of 6X His-tagged espin constructs  to GST-profilin IIa, GST-profilin I, or GST in a pull-down assay.	bind
14667	2	4993	5	NULL	NULL	0	NULL	espin constructs	NULL	6X His-tagged	bind	NULL				GST-profilin I	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_163_5_1045_s_175	14657236	(D) Binding of 6X His-tagged espin constructs  to GST-profilin IIa, GST-profilin I, or GST in a pull-down assay.	bind
14668	3	4993	5	NULL	NULL	0	NULL	espin constructs	NULL	6X His-tagged	bind	NULL				GST	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_163_5_1045_s_175	14657236	(D) Binding of 6X His-tagged espin constructs  to GST-profilin IIa, GST-profilin I, or GST in a pull-down assay.	bind
14669	4	4993	5	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_163_5_1045_s_175	14657236	(D) Binding of 6X His-tagged espin constructs  to GST-profilin IIa, GST-profilin I, or GST in a pull-down assay.	bind
14670	5	4993	5	NULL	NULL	0	NULL	statement 2	NULL		is an alternative to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_163_5_1045_s_175	14657236	(D) Binding of 6X His-tagged espin constructs  to GST-profilin IIa, GST-profilin I, or GST in a pull-down assay.	bind
13209	1	4993	6	NULL	NULL	NULL	NULL	espin constructs	GP	His-tagged	bind					GST-profilin IIa	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_163_5_1045_s_175	14657236	(D) Binding of 6X His-tagged espin constructs  to GST-profilin IIa, GST-profilin I, or GST in a pull-down assay.	bind
13210	2	4993	6	NULL	NULL	NULL	NULL	epsin constructs	GP	His-tagged	bind					GST-profilin I	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_163_5_1045_s_175	14657236	(D) Binding of 6X His-tagged espin constructs  to GST-profilin IIa, GST-profilin I, or GST in a pull-down assay.	bind
13211	3	4993	6	NULL	NULL	NULL	NULL	epsin constructs	GP	His-tagged	bind					GST					NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_163_5_1045_s_175	14657236	(D) Binding of 6X His-tagged espin constructs  to GST-profilin IIa, GST-profilin I, or GST in a pull-down assay.	bind
54624	4	4993	6	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_163_5_1045_s_175	14657236	(D) Binding of 6X His-tagged espin constructs  to GST-profilin IIa, GST-profilin I, or GST in a pull-down assay.	bind
54625	5	4993	6	NULL	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_163_5_1045_s_175	14657236	(D) Binding of 6X His-tagged espin constructs  to GST-profilin IIa, GST-profilin I, or GST in a pull-down assay.	bind
14671	1	4994	5	10	NULL	0	NULL	ornithodorin	NULL		is a type of	NULL				thrombin inhibitor	NULL	soft tick 			NULL		NULL	NULL	NULL	NULL	gw70_insectbiochemmolbiol_34_1_1_s_293	14723893	(d) Binding of a soft tick thrombin inhibitor  (ornithodorin) with thrombin ( [ Van de Locht et al., 1996]).	bind
14672	2	4994	5	NULL	NULL	0	NULL	ornithodorin	NULL		bind	NULL				thrombin	NULL				NULL		0	NULL	NULL	NULL	gw70_insectbiochemmolbiol_34_1_1_s_293	14723893	(d) Binding of a soft tick thrombin inhibitor  (ornithodorin) with thrombin ( [ Van de Locht et al., 1996]).	bind
13212	1	4994	6	NULL	NULL	NULL	NULL	ornithodorin	GP		bind					thrombin	GP				NULL		NULL	NULL	NULL	NULL	gw70_insectbiochemmolbiol_34_1_1_s_293	14723893	(d) Binding of a soft tick thrombin inhibitor  (ornithodorin) with thrombin ( [ Van de Locht et al., 1996]).	bind
13213	2	4994	6	NULL	NULL	NULL	NULL	ornithodorin	GP		is a type of					thrombin inhibitor	GP	soft tick			NULL		NULL	NULL	NULL	NULL	gw70_insectbiochemmolbiol_34_1_1_s_293	14723893	(d) Binding of a soft tick thrombin inhibitor  (ornithodorin) with thrombin ( [ Van de Locht et al., 1996]).	bind
14673	1	4995	5	NULL	NULL	0	NULL	C/EBPbeta	NULL		bind	NULL				p40	NULL	endogenous		promoter	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_6_2385_s_177	14993278	(D) Binding of C/EBPbeta to the endogenous p40 promoter was monitored  by ChIP and semiquantitative PCR by using C/EBPbeta and GST antibodies and chromatin  samples as described in the legend to Fig.  2.	bind
13214	1	4995	6	NULL	NULL	NULL	NULL	C/EBPbeta	GP		bind					p40	GP	endogenous		promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_6_2385_s_177	14993278	(D) Binding of C/EBPbeta to the endogenous p40 promoter was monitored  by ChIP and semiquantitative PCR by using C/EBPbeta and GST antibodies and chromatin  samples as described in the legend to Fig.  2.	bind
14674	1	4996	5	NULL	NULL	0	NULL	Ce-Sema1aadeltaC-Fc-AP	NULL		bind	NULL				PLX-1	NULL				NULL		0	NULL	NULL	NULL	gw60_development_129_9_2053_s_239	11959816	(D) Binding of Ce-Sema1aadeltaC-Fc-AP to PLX-1.	bind
13215	1	4996	6	NULL	NULL	NULL	NULL	Ce-Sema1aadeltaC-Fc-AP	GP		bind					PLX-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_development_129_9_2053_s_239	11959816	(D) Binding of Ce-Sema1aadeltaC-Fc-AP to PLX-1.	bind
14675	1	4997	5	NULL	NULL	0	NULL	CPEB	NULL		bind	NULL				XPum	NULL		Puf		NULL		0	NULL	NULL	NULL	gw70_mechdev_120_8_865_s_84	12963108	(D) Binding of CPEB to XPum Puf as revealed by anti-CPEB  immunoprecipitation.	bind
13216	1	4997	6	NULL	NULL	NULL	NULL	CPEB	GP		bind					Xpum	GP		puf		NULL		NULL	NULL	NULL	NULL	gw70_mechdev_120_8_865_s_84	12963108	(D) Binding of CPEB to XPum Puf as revealed by anti-CPEB  immunoprecipitation.	bind
14676	1	4998	5	NULL	NULL	0	NULL	fl- -SsrA	NULL		bind	NULL				hexameric ClpA	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_9_3_673_s_145	11931773	(D) Binding of fl- -SsrA to hexameric ClpA is inhibited by ClpS.	bind
14677	2	4998	5	NULL	NULL	0	NULL	ClpS	NULL		inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_9_3_673_s_145	11931773	(D) Binding of fl- -SsrA to hexameric ClpA is inhibited by ClpS.	bind
13217	1	4998	6	NULL	NULL	NULL	NULL	fl- -SsrA 	GP		bind					hexameric ClpA	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_9_3_673_s_145	11931773	(D) Binding of fl- -SsrA to hexameric ClpA is inhibited by ClpS.	bind
13218	2	4998	6	NULL	NULL	NULL	NULL	ClpS	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_9_3_673_s_145	11931773	(D) Binding of fl- -SsrA to hexameric ClpA is inhibited by ClpS.	bind
14678	1	4999	5	NULL	NULL	0	NULL	gp82 proteins	NULL	recombinant	bind	NULL				HeLa cells	NULL				NULL		0	NULL	NULL	NULL	gw70_microbesinfect_8_6_1502_s_102	16697683	(D) Binding of gp82 recombinant proteins to HeLa cells.	bind
13219	1	4999	6	NULL	NULL	NULL	NULL	gp82 proteins	GP	recombinant	bind					HeLa cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_microbesinfect_8_6_1502_s_102	16697683	(D) Binding of gp82 recombinant proteins to HeLa cells.	bind
14679	1	5000	5	NULL	NULL	0	NULL	GSK-3beta	NULL		bind	NULL				NEMO	NULL				NULL	extracts of astrocytes	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_13_4649_s_271	12808104	(D) Binding of GSK-3beta to NEMO was analyzed using extracts  of astrocytes.	bind
13220	1	5000	6	NULL	NULL	NULL	NULL	GSK-3beta	GP		bind					NEMO	GP				NULL	extracts of astrocytes	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_13_4649_s_271	12808104	(D) Binding of GSK-3beta to NEMO was analyzed using extracts  of astrocytes.	bind
13338	1	5001	7	NULL	NULL	0	NULL	GSK-3beta	NULL		bind	NULL				NEMO	NULL				NULL	extracts of astrocytes	0	NULL	NULL	NULL	gw60_molcellbiol_23_13_4649_s_271	12808104	(D) Binding of GSK-3beta to NEMO was analyzed using extracts of astrocytes.	bind
13222	1	5002	6	NULL	NULL	NULL	NULL	KSR	GP		bind					MEK	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5523_s_323	10409742	(D) Binding of KSR to MEK does not alter the ability of MEK to activate ERK in response to growth factor stimulation.	bind
13223	2	5002	6	NULL	NULL	NULL	NULL	MEK	GP		activate					ERK	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5523_s_323	10409742	(D) Binding of KSR to MEK does not alter the ability of MEK to activate ERK in response to growth factor stimulation.	bind
13224	3	5002	6	NULL	NULL	NULL	NULL	statement 2	Process		occurs in response to					growth factor 	GP	stimulation of 			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5523_s_323	10409742	(D) Binding of KSR to MEK does not alter the ability of MEK to activate ERK in response to growth factor stimulation.	bind
17351	4	5002	6	NULL	NULL	NULL	NULL	statement 1	Process		does not alter					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5523_s_323	10409742	(D) Binding of KSR to MEK does not alter the ability of MEK to activate ERK in response to growth factor stimulation.	bind
13339	1	5002	7	NULL	NULL	0	NULL	 KSR 	NULL		bind	NULL				MEK	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_8_5523_s_323	10409742	(D) Binding of KSR to MEK does not alter the ability of MEK to activate ERK in response to growth factor stimulation.	bind
13340	2	5002	7	NULL	NULL	0	NULL	MEK	NULL		activate	NULL				ERK	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5523_s_323	10409742	(D) Binding of KSR to MEK does not alter the ability of MEK to activate ERK in response to growth factor stimulation.	bind
13341	3	5002	7	NULL	NULL	0	NULL	statement 2	NULL		occurs in response to	NULL				growth factor	NULL	stimulation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5523_s_323	10409742	(D) Binding of KSR to MEK does not alter the ability of MEK to activate ERK in response to growth factor stimulation.	bind
13342	4	5002	7	NULL	NULL	0	NULL	statement 1	NULL		does not alter	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_8_5523_s_323	10409742	(D) Binding of KSR to MEK does not alter the ability of MEK to activate ERK in response to growth factor stimulation.	bind
13225	1	5003	6	NULL	NULL	NULL	NULL	MCP-1 variants	GP		bind					M3	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_111_3_343_s_163	12419245	(D) Binding of MCP-1 variants to M3.	bind
13343	1	5003	7	NULL	NULL	0	NULL	MCP-1 variants	NULL		bind	NULL				M3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cell_111_3_343_s_163	12419245	(D) Binding of MCP-1 variants to M3.	bind
13226	1	5004	6	NULL	NULL	NULL	NULL	p27	GP		bind					Cdk2 complexes	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_1_55_s_74	15631990	(D) Binding of p27 to Cdk2  complexes.	bind
13344	1	5004	7	NULL	NULL	0	NULL	p27	NULL		bind	NULL				Cdk2 complex	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_168_1_55_s_74	15631990	(D) Binding of p27 to Cdk2  complexes.	bind
13227	1	5005	6	NULL	NULL	NULL	NULL	peptidyl-tRNA	NucleicAcid		bind							classical	P site		NULL		NULL	NULL	NULL	NULL	gw60_structure_4_3_229_s_277	8805530	(d) Binding of peptidyl-tRNA and aminoacyl-tRNA in classical P and A sites.	bind
13228	2	5005	6	NULL	NULL	NULL	NULL	aminoacyl-tRNA	NucleicAcid		bind							classical	A site		NULL		NULL	NULL	NULL	NULL	gw60_structure_4_3_229_s_277	8805530	(d) Binding of peptidyl-tRNA and aminoacyl-tRNA in classical P and A sites.	bind
13345	1	5005	7	NULL	NULL	0	NULL	peptidyl-tRNA	NULL		bind	NULL					NULL	classical	P site		NULL		NULL	NULL	NULL	NULL	gw60_structure_4_3_229_s_277	8805530	(d) Binding of peptidyl-tRNA and aminoacyl-tRNA in classical P and A sites.	bind
13348	4	5005	7	NULL	NULL	0	NULL	aminoacyl-tRNA	NULL		bind	NULL					NULL	classical	A site		NULL		0	NULL	NULL	NULL	gw60_structure_4_3_229_s_277	8805530	(d) Binding of peptidyl-tRNA and aminoacyl-tRNA in classical P and A sites.	bind
13258	1	5006	6	NULL	NULL	NULL	NULL	pp90RSK	GP		bind					p300	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_86_3_465_s_110	8756728	(d) Binding of pp90RSK to  P300 does not interfere with binding of phospho-CREB to P300.	bind
13259	2	5006	6	NULL	NULL	NULL	NULL	phospho-CREB	GP		bind					p300	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_86_3_465_s_110	8756728	(d) Binding of pp90RSK to  P300 does not interfere with binding of phospho-CREB to P300.	bind
13260	3	5006	6	NULL	NULL	NULL	NULL	statement 1	Process		does not interfere with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_86_3_465_s_110	8756728	(d) Binding of pp90RSK to  P300 does not interfere with binding of phospho-CREB to P300.	bind
13349	1	5006	7	NULL	NULL	0	NULL	phospho-CREB	NULL		bind	NULL				P300	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cell_86_3_465_s_110	8756728	(d) Binding of pp90RSK to  P300 does not interfere with binding of phospho-CREB to P300.	bind
13350	2	5006	7	NULL	NULL	0	NULL	pp90RSK	NULL		bind	NULL				P300	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_86_3_465_s_110	8756728	(d) Binding of pp90RSK to  P300 does not interfere with binding of phospho-CREB to P300.	bind
13351	3	5006	7	NULL	NULL	0	NULL	statement 2	NULL		does not interfere with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_86_3_465_s_110	8756728	(d) Binding of pp90RSK to  P300 does not interfere with binding of phospho-CREB to P300.	bind
13261	1	5007	6	NULL	NULL	NULL	NULL	GRASP55	GP	purified	bind					p24 proteins	GP		cytoplasmic tail		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_68	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the cytoplasmic tails of the various p24 proteins, TGF-alpha, and GM130.	bind
13262	2	5007	6	NULL	NULL	NULL	NULL	GRASP55	GP	purified	bind					TGF-alpha	GP		cytoplasmic tail		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_68	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the cytoplasmic tails of the various p24 proteins, TGF-alpha, and GM130.	bind
13263	3	5007	6	NULL	NULL	NULL	NULL	GRASP55	GP	purified	bind					GM130	GP		cytoplasmic tail		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_68	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the cytoplasmic tails of the various p24 proteins, TGF-alpha, and GM130.	bind
13264	4	5007	6	NULL	NULL	NULL	NULL	GRASP65	GP	purified	bind					p24 proteins	GP		cytoplasmic tail		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_68	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the cytoplasmic tails of the various p24 proteins, TGF-alpha, and GM130.	bind
13265	5	5007	6	NULL	NULL	NULL	NULL	GRASP65	GP	purified	bind					TGF-alpha	GP		cytoplasmic tail		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_68	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the cytoplasmic tails of the various p24 proteins, TGF-alpha, and GM130.	bind
13266	6	5007	6	NULL	NULL	NULL	NULL	GRASP65	GP	purified	bind					GM130	GP		cytoplasmic tail		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_68	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the cytoplasmic tails of the various p24 proteins, TGF-alpha, and GM130.	bind
44615	7	5007	6	NULL	NULL	NULL	NULL	p24 proteins	GP		is a type of					GST fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_68	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the cytoplasmic tails of the various p24 proteins, TGF-alpha, and GM130.	bind
44617	8	5007	6	NULL	NULL	NULL	NULL	TGF-alpha	GP		is a type of					GST fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_68	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the cytoplasmic tails of the various p24 proteins, TGF-alpha, and GM130.	bind
44620	9	5007	6	NULL	NULL	NULL	NULL	GM130	GP		is a type of					GST fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_68	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the cytoplasmic tails of the various p24 proteins, TGF-alpha, and GM130.	bind
13352	1	5007	7	10	NULL	0	NULL	GRASP55	NULL	purified	bind	NULL				p24 protein	NULL		cytoplasmic tails		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_68	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the cytoplasmic tails of the various p24 proteins, TGF-alpha, and GM130.	bind
13353	2	5007	7	10	NULL	0	NULL	GRASP55	NULL	purified	bind	NULL				TGF-alpha	NULL		cytoplasmic tails		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_68	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the cytoplasmic tails of the various p24 proteins, TGF-alpha, and GM130.	bind
13354	3	5007	7	10	NULL	0	NULL	GRASP55	NULL	purified	bind	NULL				GM130	NULL		cytoplasmic tails		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_68	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the cytoplasmic tails of the various p24 proteins, TGF-alpha, and GM130.	bind
13355	4	5007	7	10	NULL	0	NULL	GRASP65	NULL	purified	bind	NULL				p24 protein	NULL		cytoplasmic tails		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_68	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the cytoplasmic tails of the various p24 proteins, TGF-alpha, and GM130.	bind
13356	5	5007	7	10	NULL	0	NULL	GRASP65	NULL	purified	bind	NULL				TGF-alpha	NULL		cytoplasmic tails		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_68	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the cytoplasmic tails of the various p24 proteins, TGF-alpha, and GM130.	bind
13357	6	5007	7	10	NULL	0	NULL	GRASP65	NULL	purified	bind	NULL				GM130	NULL		cytoplasmic tails		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_68	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the cytoplasmic tails of the various p24 proteins, TGF-alpha, and GM130.	bind
44616	7	5007	7	10	NULL	0	NULL	p24 proteins	NULL		is a type of	NULL				GST fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_68	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the cytoplasmic tails of the various p24 proteins, TGF-alpha, and GM130.	bind
44619	8	5007	7	10	NULL	0	NULL	TGF-alpha	NULL		is a type of	NULL				GST fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_68	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the cytoplasmic tails of the various p24 proteins, TGF-alpha, and GM130.	bind
44621	9	5007	7	10	NULL	0	NULL	GM130	NULL		is a type of	NULL				GST fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_68	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the cytoplasmic tails of the various p24 proteins, TGF-alpha, and GM130.	bind
13267	1	5008	6	NULL	NULL	NULL	NULL	GRASP55	GP	purified	bind					p24a	GP	wild-type	cytoplasmic tail		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_82	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the wild-type and point mutant forms of the p24a cytoplasmic tail, and GM130.	bind
13268	2	5008	6	NULL	NULL	NULL	NULL	Grasp55	GP	purified	bind					GM130	GP	wild-type			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_82	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the wild-type and point mutant forms of the p24a cytoplasmic tail, and GM130.	bind
13269	3	5008	6	NULL	NULL	NULL	NULL	GRASP55	GP	purified	bind					p24a	GP	point mutant	cytoplasmic tail		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_82	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the wild-type and point mutant forms of the p24a cytoplasmic tail, and GM130.	bind
13270	4	5008	6	NULL	NULL	NULL	NULL	GRASP55	GP	purified	bind					GM130	GP	point mutant			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_82	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the wild-type and point mutant forms of the p24a cytoplasmic tail, and GM130.	bind
17352	5	5008	6	NULL	NULL	NULL	NULL	GRASP65	GP	purified	bind					p24a	GP	wild-type	cytoplasmic tail		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_82	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the wild-type and point mutant forms of the p24a cytoplasmic tail, and GM130.	bind
17353	6	5008	6	NULL	NULL	NULL	NULL	GRASP65	GP	purified	bind					GM130	GP	wild-type			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_82	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the wild-type and point mutant forms of the p24a cytoplasmic tail, and GM130.	bind
17354	7	5008	6	NULL	NULL	NULL	NULL	GRASP65	GP	purified	bind					p24a	GP	point mutant	cytoplasmic tail		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_82	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the wild-type and point mutant forms of the p24a cytoplasmic tail, and GM130.	bind
17355	8	5008	6	NULL	NULL	NULL	NULL	GRASP65	GP	purified	bind					GM130	GP	point mutant			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_82	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the wild-type and point mutant forms of the p24a cytoplasmic tail, and GM130.	bind
44622	9	5008	6	NULL	NULL	NULL	NULL	p24a	GP		is a type of					GST fusion protein					NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_82	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the wild-type and point mutant forms of the p24a cytoplasmic tail, and GM130.	bind
44624	10	5008	6	NULL	NULL	NULL	NULL	GM130	GP		is a type of					GST fusion protein					NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_82	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the wild-type and point mutant forms of the p24a cytoplasmic tail, and GM130.	bind
13358	1	5008	7	10	NULL	0	NULL	GRASP55	NULL	purified	bind	NULL				 p24a	NULL	wild-type	cytoplasmic tail		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_82	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the wild-type and point mutant forms of the p24a cytoplasmic tail, and GM130.	bind
13359	2	5008	7	10	NULL	0	NULL	GRASP55	NULL	purified	bind	NULL				p24a	NULL	point mutant	cytoplasmic tail		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_82	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the wild-type and point mutant forms of the p24a cytoplasmic tail, and GM130.	bind
13360	3	5008	7	10	NULL	0	NULL	GRASP55	NULL	purified	bind	NULL				GM130	NULL	wild-type			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_82	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the wild-type and point mutant forms of the p24a cytoplasmic tail, and GM130.	bind
13361	4	5008	7	10	NULL	0	NULL	GRASP55	NULL	purified	bind	NULL				GM130	NULL	point mutant			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_82	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the wild-type and point mutant forms of the p24a cytoplasmic tail, and GM130.	bind
13362	5	5008	7	10	NULL	0	NULL	GRASP65	NULL	purified	bind	NULL				p24a	NULL	wild-type	cytoplasmic tail		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_82	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the wild-type and point mutant forms of the p24a cytoplasmic tail, and GM130.	bind
13363	6	5008	7	10	NULL	0	NULL	GRASP65	NULL	purified	bind	NULL				p24a	NULL	point mutant	cytoplasmic tail		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_82	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the wild-type and point mutant forms of the p24a cytoplasmic tail, and GM130.	bind
13364	7	5008	7	10	NULL	0	NULL	GRASP65	NULL	purified	bind	NULL				GM130	NULL	wild-type			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_82	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the wild-type and point mutant forms of the p24a cytoplasmic tail, and GM130.	bind
13365	8	5008	7	10	NULL	0	NULL	GRASP65	NULL	purified	bind	NULL				GM130	NULL	point mutant			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_82	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the wild-type and point mutant forms of the p24a cytoplasmic tail, and GM130.	bind
44625	10	5008	7	10	NULL	0	NULL	GM130	NULL		is a type of	NULL				GST fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_82	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the wild-type and point mutant forms of the p24a cytoplasmic tail, and GM130.	bind
44626	9	5008	7	10	NULL	0	NULL	p24a	NULL		is a type of	NULL				GST fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_155_6_885_s_82	11739402	(D) Binding of purified GRASP55 and GRASP65 to GST fusion proteins bearing the wild-type and point mutant forms of the p24a cytoplasmic tail, and GM130.	bind
13271	1	5009	6	NULL	NULL	NULL	NULL	Rpb1	GP		bind					GAL1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_18_6270_s_216	11509669	(D) Binding of Rpb1 to the  GAL1 and  GAL10 promoters.	bind
13272	2	5009	6	NULL	NULL	NULL	NULL	Rpb1	GP		bind					GAL10	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_18_6270_s_216	11509669	(D) Binding of Rpb1 to the  GAL1 and  GAL10 promoters.	bind
13366	1	5009	7	NULL	NULL	0	NULL	Rpb1	NULL		bind	NULL				GAL1	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_18_6270_s_216	11509669	(D) Binding of Rpb1 to the  GAL1 and  GAL10 promoters.	bind
13367	2	5009	7	NULL	NULL	0	NULL	Rpb1	NULL		bind	NULL				GAL10	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_18_6270_s_216	11509669	(D) Binding of Rpb1 to the  GAL1 and  GAL10 promoters.	bind
13273	1	5010	6	NULL	NULL	NULL	NULL	Sar1p	GP		bind					Sec23/24p complex	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_3_395_s_203	11970962	(D) Binding of Sar1p and Sec23/24p complex is enhanced in the presence of Glo3p.	bind
13274	2	5010	6	NULL	NULL	NULL	NULL	Glo3p	GP		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_3_395_s_203	11970962	(D) Binding of Sar1p and Sec23/24p complex is enhanced in the presence of Glo3p.	bind
13368	1	5010	7	NULL	NULL	0	NULL	Sar1p 	NULL		bind	NULL				Sec23/24p complex	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_157_3_395_s_203	11970962	(D) Binding of Sar1p and Sec23/24p complex is enhanced in the presence of Glo3p.	bind
13369	2	5010	7	10	NULL	0	NULL	Glo3p	NULL		enhance	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_3_395_s_203	11970962	(D) Binding of Sar1p and Sec23/24p complex is enhanced in the presence of Glo3p.	bind
13275	1	5011	6	NULL	NULL	NULL	NULL	Sla2p	GP		bind					PtdIns3P	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_2_717_s_113	15574875	(D) Binding of Sla2p to PtdIns3P, PtdIns4P, and PtdIns5P.	bind
13276	2	5011	6	NULL	NULL	NULL	NULL	Sla2p	GP		bind					PtdIns4P	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_2_717_s_113	15574875	(D) Binding of Sla2p to PtdIns3P, PtdIns4P, and PtdIns5P.	bind
13277	3	5011	6	NULL	NULL	NULL	NULL	Sla2p	GP		bind					PtdIns5P	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_2_717_s_113	15574875	(D) Binding of Sla2p to PtdIns3P, PtdIns4P, and PtdIns5P.	bind
13370	1	5011	7	NULL	NULL	0	NULL	Sla2p	NULL		bind	NULL				PtdIns3P	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_2_717_s_113	15574875	(D) Binding of Sla2p to PtdIns3P, PtdIns4P, and PtdIns5P.	bind
13371	2	5011	7	NULL	NULL	0	NULL	Sla2p 	NULL		bind	NULL				PtdIns4P	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_2_717_s_113	15574875	(D) Binding of Sla2p to PtdIns3P, PtdIns4P, and PtdIns5P.	bind
13372	3	5011	7	NULL	NULL	0	NULL	Sla2p	NULL		bind	NULL				PtdIns5P	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_2_717_s_113	15574875	(D) Binding of Sla2p to PtdIns3P, PtdIns4P, and PtdIns5P.	bind
13278	1	5012	6	NULL	NULL	NULL	NULL	Synaptotagmin	GP		bind					GST-SyxH3-C	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_23_3_593_s_220	10433270	(D) Binding of Synaptotagmin to GST-SyxH3-C is strongly reduced compared to GST-Syx.	bind
13279	2	5012	6	NULL	NULL	NULL	NULL	Synaptotagmin	GP		bind					GST-Syx	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_23_3_593_s_220	10433270	(D) Binding of Synaptotagmin to GST-SyxH3-C is strongly reduced compared to GST-Syx.	bind
13280	3	5012	6	NULL	NULL	NULL	NULL	statement 1	Process		is reduced than		strongly			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_23_3_593_s_220	10433270	(D) Binding of Synaptotagmin to GST-SyxH3-C is strongly reduced compared to GST-Syx.	bind
13373	1	5012	7	NULL	NULL	0	NULL	Synaptotagmin	NULL		bind	NULL				GST-SyxH3-C	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_23_3_593_s_220	10433270	(D) Binding of Synaptotagmin to GST-SyxH3-C is strongly reduced compared to GST-Syx.	bind
13374	2	5012	7	NULL	NULL	0	NULL	Synaptotagmin	NULL		bind	NULL				GST-Syx	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_23_3_593_s_220	10433270	(D) Binding of Synaptotagmin to GST-SyxH3-C is strongly reduced compared to GST-Syx.	bind
13375	3	5012	7	10	NULL	0	NULL	statement 1	NULL		is reduced than	NULL	strongly			statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuron_23_3_593_s_220	10433270	(D) Binding of Synaptotagmin to GST-SyxH3-C is strongly reduced compared to GST-Syx.	bind
13281	1	5013	6	NULL	NULL	NULL	NULL	translation factors	GP		bind					eIF4GI	GP	point mutant			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_2_468_s_224	10611225	(D) Binding of translation factors to eIF4GI point mutants in vitro.	bind
13376	1	5013	7	NULL	NULL	0	NULL	 translation factors	NULL		bind	NULL				eIF4GI	NULL	point mutant			NULL	in vitro	0	NULL	NULL	NULL	gw60_molcellbiol_20_2_468_s_224	10611225	(D) Binding of translation factors to eIF4GI point mutants in vitro.	bind
13282	1	5015	6	NULL	NULL	NULL	NULL	TSG101	GP		bind					Hrs	GP	deletion mutant			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_162_3_425_s_83	12900394	(D) Binding of Tsg101 to Hrs deletion mutants.	bind
13377	1	5015	7	NULL	NULL	0	NULL	Tsg101	NULL		bind	NULL				Hrs	NULL	deletion mutant			NULL		0	NULL	NULL	NULL	gw60_cellbiol_162_3_425_s_83	12900394	(D) Binding of Tsg101 to Hrs deletion mutants.	bind
13283	1	5016	6	NULL	NULL	NULL	NULL	GST-Spo20p	GP	wt	bind			61-91		PA	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_4_1802_s_249	14742704	(D) Binding of wt and mutant  GST-Spo20p61-91 to PA.	bind
13284	2	5016	6	10	NULL	0	NULL	GST-Spo20p	NULL	mutant	bind	NULL		61-91		PA	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_4_1802_s_249	14742704	(D) Binding of wt and mutant  GST-Spo20p61-91 to PA.	bind
13378	1	5016	7	10	NULL	0	NULL	GST-Spo20p	NULL	wt	bind	NULL		61-91		PA	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_4_1802_s_249	14742704	(D) Binding of wt and mutant  GST-Spo20p61-91 to PA.	bind
13379	2	5016	7	10	NULL	0	NULL	GST-Spo20p	NULL	mutant	bind	NULL		61-91		PA	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_4_1802_s_249	14742704	(D) Binding of wt and mutant  GST-Spo20p61-91 to PA.	bind
13285	1	5017	6	NULL	NULL	NULL	NULL	Xrn1p	GP		bind					actin RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_5930_s_244	10454540	(D) Binding of Xrn1p and Xrn1-D208Ap to actin RNA (nuclease substrate of panel C) was determined by filter binding.	bind
13286	2	5017	6	NULL	NULL	NULL	NULL	Xrn1	GP		bind			D208Ap		actin RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_5930_s_244	10454540	(D) Binding of Xrn1p and Xrn1-D208Ap to actin RNA (nuclease substrate of panel C) was determined by filter binding.	bind
13380	1	5017	7	NULL	NULL	0	NULL	Xrn1p	NULL		bind	NULL				actin RNA	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_5930_s_244	10454540	(D) Binding of Xrn1p and Xrn1-D208Ap to actin RNA (nuclease substrate of panel C) was determined by filter binding.	bind
13381	2	5017	7	NULL	NULL	0	NULL	Xrn1p	NULL		bind	NULL		D208A		actin RNA	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_5930_s_244	10454540	(D) Binding of Xrn1p and Xrn1-D208Ap to actin RNA (nuclease substrate of panel C) was determined by filter binding.	bind
13287	1	5018	6	NULL	NULL	NULL	NULL				bind			RGG box		sc1 RNAs	NucleicAcid	truncated	bp 1 - 58		NULL		NULL	NULL	NULL	NULL	gw60_cell_107_4_489_s_144	11719189	(D) Binding specificity  of the RGG box (cterm 10) to truncated  sc1 RNAs (bp 1 - 58), or mutants G37-G38 or  G42-G43 to CC.	bind
13382	1	5018	7	NULL	NULL	0	NULL		NULL		bind	NULL		RGG box 		sc1 RNAs	NULL	truncated	bp 1 - 58		NULL		NULL	NULL	NULL	NULL	gw60_cell_107_4_489_s_144	11719189	(D) Binding specificity  of the RGG box (cterm 10) to truncated  sc1 RNAs (bp 1 - 58), or mutants G37-G38 or  G42-G43 to CC.	bind
13288	1	5019	6	NULL	NULL	NULL	NULL	RXR-VDR heterodimer	GP		bind							specific		VDRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_257	10891484	(D) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-VDR heterodimer bound to a specific VDRE.	bind
13289	2	5019	6	NULL	NULL	NULL	NULL	TRAP220	GP		bind		efficiently	RBD		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_257	10891484	(D) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-VDR heterodimer bound to a specific VDRE.	bind
13290	3	5019	6	NULL	NULL	NULL	NULL			proper spacing of 	is necessary for			RBD-1		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_257	10891484	(D) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-VDR heterodimer bound to a specific VDRE.	bind
17356	4	5019	6	NULL	NULL	NULL	NULL			proper spacing of	is necessary for			RBD-2		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_257	10891484	(D) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-VDR heterodimer bound to a specific VDRE.	bind
44711	5	5019	6	NULL	NULL	NULL	NULL			presence of	is necessary for			RBD-1		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_257	10891484	(D) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-VDR heterodimer bound to a specific VDRE.	bind
44712	6	5019	6	NULL	NULL	NULL	NULL			presence of	is necessary for			RBD-2		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_257	10891484	(D) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-VDR heterodimer bound to a specific VDRE.	bind
13384	1	5019	7	NULL	NULL	0	NULL	RXR-VDR heterodimer	NULL		bind	NULL					NULL	specific		VDRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_257	10891484	(D) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-VDR heterodimer bound to a specific VDRE.	bind
13385	2	5019	7	NULL	NULL	0	NULL	TRAP220	NULL		bind	NULL	efficiently	RBD		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_257	10891484	(D) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-VDR heterodimer bound to a specific VDRE.	bind
13386	3	5019	7	NULL	NULL	0	NULL		NULL	proper spacing of	is necessary for	NULL		RBD-1		statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_257	10891484	(D) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-VDR heterodimer bound to a specific VDRE.	bind
13387	4	5019	7	NULL	NULL	0	NULL		NULL	proper spacing of	is necessary for	NULL		RBD-2		statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_257	10891484	(D) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-VDR heterodimer bound to a specific VDRE.	bind
44717	5	5019	7	NULL	NULL	0	NULL		NULL	presence of	is necessary for	NULL		RBD-1		statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_257	10891484	(D) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-VDR heterodimer bound to a specific VDRE.	bind
44718	6	5019	7	NULL	NULL	0	NULL		NULL	presence of 	is necessary for	NULL		RBD-2		statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_15_5433_s_257	10891484	(D) Both the presence and proper spacing of RBD-1 and RBD-2 are necessary for efficient binding of TRAP220 RBD to an RXR-VDR heterodimer bound to a specific VDRE.	bind
13291	1	5020	6	NULL	NULL	NULL	NULL	eIF4G	GP		bind					Mnk2a	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_16_5692_s_289	12897141	(D) C-terminal deletions affect binding of eIF4G to Mnk2a.	bind
13292	2	5020	6	NULL	NULL	NULL	NULL			deletion of	affect			C-terminus		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_16_5692_s_289	12897141	(D) C-terminal deletions affect binding of eIF4G to Mnk2a.	bind
13388	1	5020	7	NULL	NULL	0	NULL	eIF4G	NULL		bind	NULL				Mnk2a	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_16_5692_s_289	12897141	(D) C-terminal deletions affect binding of eIF4G to Mnk2a.	bind
13389	2	5020	7	NULL	NULL	0	NULL		NULL	deletion of	affect	NULL		C-terminal 		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_16_5692_s_289	12897141	(D) C-terminal deletions affect binding of eIF4G to Mnk2a.	bind
13293	1	5021	6	NULL	NULL	NULL	NULL	C4BP	GP		bind		directly			CD40	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_18_6_837_s_46	12818164	(D) C4BP  binds directly to CD40.	bind
13390	1	5021	7	NULL	NULL	0	NULL	C4BP	NULL		binds	NULL	directly			CD40	NULL				NULL		0	NULL	NULL	NULL	gw60_immunity_18_6_837_s_46	12818164	(D) C4BP  binds directly to CD40.	bind
13294	1	5022	6	NULL	NULL	NULL	NULL	myosin-Va	GP		bind					syntaxin-1A	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_96	16030255	(D) Ca2+-dependence of myosin-Va binding to syntaxin-1A.	bind
13295	2	5022	6	NULL	NULL	NULL	NULL	statement 1	Process		is dependent on					Ca+2	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_96	16030255	(D) Ca2+-dependence of myosin-Va binding to syntaxin-1A.	bind
13391	1	5022	7	NULL	NULL	0	NULL	myosin-Va	NULL		bind	NULL				syntaxin-1A	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_96	16030255	(D) Ca2+-dependence of myosin-Va binding to syntaxin-1A.	bind
13392	2	5022	7	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				Ca2+	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_96	16030255	(D) Ca2+-dependence of myosin-Va binding to syntaxin-1A.	bind
13296	1	5023	6	NULL	NULL	NULL	NULL	CAML	GP		does not bind					FGFR1	GP				NULL	PC-12 cells	NULL	NULL	NULL	NULL	gw60_devcell_5_2_245_s_154	12919676	(D) CAML does not bind the FGFR1 in PC-12 cells.	bind
13393	1	5023	7	NULL	NULL	0	NULL	CAML	NULL		does not bind	NULL				FGFR1	NULL				NULL	PC-12 cells	0	NULL	NULL	NULL	gw60_devcell_5_2_245_s_154	12919676	(D) CAML does not bind the FGFR1 in PC-12 cells.	bind
13297	1	5025	6	NULL	NULL	NULL	NULL	Cdc24	GP		bind			FW253AA		Pcn1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_2_1038_s_235	9891039	(D) Cdc24(FW253AA) binds Pcn1 and Rfc1.	bind
13298	2	5025	6	NULL	NULL	NULL	NULL	Cdc24	GP		bind			FW253AA		Rfc1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_2_1038_s_235	9891039	(D) Cdc24(FW253AA) binds Pcn1 and Rfc1.	bind
13394	1	5025	7	NULL	NULL	0	NULL	Cdc24	NULL		binds	NULL		FW253AA		Pcn1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_2_1038_s_235	9891039	(D) Cdc24(FW253AA) binds Pcn1 and Rfc1.	bind
13395	2	5025	7	NULL	NULL	0	NULL	 Cdc24	NULL		binds	NULL		FW253AA		Rfc1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_2_1038_s_235	9891039	(D) Cdc24(FW253AA) binds Pcn1 and Rfc1.	bind
13299	1	5027	6	NULL	NULL	NULL	NULL	SF-1	GP	endogenous	bind		directly			Oct4	GP			PE	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_9_3492_s_150	15831456	(D) ChIP analysis of direct binding of endogenous  SF-1 and LRH-1 to the Oct4 PE and PP in vivo.	bind
13300	2	5027	6	NULL	NULL	NULL	NULL	SF-1	GP	endogenous	bind		directly			Oct4	GP			PP	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_9_3492_s_150	15831456	(D) ChIP analysis of direct binding of endogenous  SF-1 and LRH-1 to the Oct4 PE and PP in vivo.	bind
13301	3	5027	6	NULL	NULL	NULL	NULL	LRH-1	GP	endogenous	bind		directly			Oct4	GP			PE	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_9_3492_s_150	15831456	(D) ChIP analysis of direct binding of endogenous  SF-1 and LRH-1 to the Oct4 PE and PP in vivo.	bind
13302	4	5027	6	NULL	NULL	NULL	NULL	LRH-1	GP	endogenous	bind		directly			Oct4	GP			PP	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_9_3492_s_150	15831456	(D) ChIP analysis of direct binding of endogenous  SF-1 and LRH-1 to the Oct4 PE and PP in vivo.	bind
13396	1	5027	7	NULL	NULL	0	NULL	SF-1	NULL	endogenous	binds	NULL	directly			Oct4	NULL			PE	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_9_3492_s_150	15831456	(D) ChIP analysis of direct binding of endogenous  SF-1 and LRH-1 to the Oct4 PE and PP in vivo.	bind
13397	2	5027	7	NULL	NULL	0	NULL	SF-1	NULL	endogenous	binds	NULL	directly			Oct4	NULL			PP	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_9_3492_s_150	15831456	(D) ChIP analysis of direct binding of endogenous  SF-1 and LRH-1 to the Oct4 PE and PP in vivo.	bind
13398	3	5027	7	NULL	NULL	0	NULL	LRH-1	NULL	endogenous	binds	NULL	directly			Oct4 	NULL			PE	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_9_3492_s_150	15831456	(D) ChIP analysis of direct binding of endogenous  SF-1 and LRH-1 to the Oct4 PE and PP in vivo.	bind
13399	4	5027	7	NULL	NULL	0	NULL	LRH-1	NULL	endogenous	binds	NULL	directly			Oct4	NULL			PP	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_9_3492_s_150	15831456	(D) ChIP analysis of direct binding of endogenous  SF-1 and LRH-1 to the Oct4 PE and PP in vivo.	bind
13303	1	5028	6	NULL	NULL	NULL	NULL	PDX-1	GP	endogenous	bind					LRH-1	GP	human		promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_19_6713_s_161	12972592	(D) ChIP assay demonstrating binding of endogenous PDX-1  to the human LRH-1 promoter.	bind
13400	1	5028	7	NULL	NULL	0	NULL	PDX-1	NULL	endogenous	bind	NULL				LRH-1	NULL	human		promoter	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_19_6713_s_161	12972592	(D) ChIP assay demonstrating binding of endogenous PDX-1  to the human LRH-1 promoter.	bind
13304	1	5029	6	NULL	NULL	NULL	NULL	Runx2	GP	endogenous	bind					beta-casein	GP	endogenous		promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3182_s_152	15798204	(D) ChIP assay demonstrating the binding of endogenous Runx2 and Oct-1  to the endogenous beta-casein promoter.	bind
13305	2	5029	6	NULL	NULL	NULL	NULL	Oct-1	GP	endogenous	bind					beta-casein	GP	endogenous		promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3182_s_152	15798204	(D) ChIP assay demonstrating the binding of endogenous Runx2 and Oct-1  to the endogenous beta-casein promoter.	bind
13401	1	5029	7	NULL	NULL	0	NULL	Runx2	NULL	endogenous	bind	NULL				beta-casein	NULL	endogenous		promoter	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_8_3182_s_152	15798204	(D) ChIP assay demonstrating the binding of endogenous Runx2 and Oct-1  to the endogenous beta-casein promoter.	bind
13402	2	5029	7	NULL	NULL	0	NULL	Oct-1	NULL	endogenous	bind	NULL				beta-casein	NULL	endogenous		promoter	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_8_3182_s_152	15798204	(D) ChIP assay demonstrating the binding of endogenous Runx2 and Oct-1  to the endogenous beta-casein promoter.	bind
13306	1	5030	6	NULL	NULL	NULL	NULL	AP-1	GP		bind					hTERT	GP			promoter	NULL	in vivo using HeLa cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_18_8037_s_165	16135795	(D) ChIP assay to verify the  binding of AP-1 to the  hTERT promoter in vivo using HeLa cells.	bind
13404	1	5030	7	10	NULL	0	NULL	AP-1	NULL		bind	NULL				hTERT	NULL			promoter	NULL	in vivo using HeLa cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_18_8037_s_165	16135795	(D) ChIP assay to verify the  binding of AP-1 to the  hTERT promoter in vivo using HeLa cells.	bind
13307	1	5031	6	NULL	NULL	NULL	NULL	RB	GP		bind					LPL	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_6_903_s_113	12479814	(D) Chromatin immunoprecipitation (ChIP) assays demonstrating binding of RB, PPAR , or HDAC3 to the LPL promoter.	bind
13308	2	5031	6	NULL	NULL	NULL	NULL	PPAR	GP		bind					LPL	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_6_903_s_113	12479814	(D) Chromatin immunoprecipitation (ChIP) assays demonstrating binding of RB, PPAR , or HDAC3 to the LPL promoter.	bind
13309	3	5031	6	NULL	NULL	NULL	NULL	HDAC3	GP		bind					LPL	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_6_903_s_113	12479814	(D) Chromatin immunoprecipitation (ChIP) assays demonstrating binding of RB, PPAR , or HDAC3 to the LPL promoter.	bind
13310	4	5031	6	NULL	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_6_903_s_113	12479814	(D) Chromatin immunoprecipitation (ChIP) assays demonstrating binding of RB, PPAR , or HDAC3 to the LPL promoter.	bind
44713	5	5031	6	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_6_903_s_113	12479814	(D) Chromatin immunoprecipitation (ChIP) assays demonstrating binding of RB, PPAR , or HDAC3 to the LPL promoter.	bind
13405	1	5031	7	NULL	NULL	0	NULL	 RB	NULL		bind	NULL				LPL	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_devcell_3_6_903_s_113	12479814	(D) Chromatin immunoprecipitation (ChIP) assays demonstrating binding of RB, PPAR , or HDAC3 to the LPL promoter.	bind
13409	2	5031	7	NULL	NULL	0	NULL	PPAR	NULL		bind	NULL				LPL	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_devcell_3_6_903_s_113	12479814	(D) Chromatin immunoprecipitation (ChIP) assays demonstrating binding of RB, PPAR , or HDAC3 to the LPL promoter.	bind
13410	3	5031	7	NULL	NULL	0	NULL	HDAC3	NULL		bind	NULL				LPL	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_devcell_3_6_903_s_113	12479814	(D) Chromatin immunoprecipitation (ChIP) assays demonstrating binding of RB, PPAR , or HDAC3 to the LPL promoter.	bind
44719	4	5031	7	NULL	NULL	0	NULL	statement 2	NULL		is an alternative to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_devcell_3_6_903_s_113	12479814	(D) Chromatin immunoprecipitation (ChIP) assays demonstrating binding of RB, PPAR , or HDAC3 to the LPL promoter.	bind
53049	5	5031	7	10	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_devcell_3_6_903_s_113	12479814	(D) Chromatin immunoprecipitation (ChIP) assays demonstrating binding of RB, PPAR , or HDAC3 to the LPL promoter.	bind
13311	1	5032	6	NULL	NULL	NULL	NULL	MEF	GP		bind					PFP	GP			promoter	NULL	PFP-positive CTLL-2 cell line	NULL	NULL	NULL	NULL	gw60_immunity_17_4_437_s_194	12387738	(D) Chromatin immunoprecipitation analysis of MEF binding to PFP promoter in the PFP-positive CTLL-2 cell line but not the PFP-negative EL-4 cell line.	bind
13312	2	5032	6	NULL	NULL	NULL	NULL	MEF	GP		does not bind					PFP	GP			promoter	NULL	PFP-negative EL-4 cell line	NULL	NULL	NULL	NULL	gw60_immunity_17_4_437_s_194	12387738	(D) Chromatin immunoprecipitation analysis of MEF binding to PFP promoter in the PFP-positive CTLL-2 cell line but not the PFP-negative EL-4 cell line.	bind
13411	1	5032	7	NULL	NULL	0	NULL	MEF	NULL		bind	NULL				PFP	NULL			promoter	NULL	PFP-positive CTLL-2 cell line	NULL	NULL	NULL	NULL	gw60_immunity_17_4_437_s_194	12387738	(D) Chromatin immunoprecipitation analysis of MEF binding to PFP promoter in the PFP-positive CTLL-2 cell line but not the PFP-negative EL-4 cell line.	bind
13412	2	5032	7	NULL	NULL	0	NULL	MEF	NULL		does not bind	NULL				PFP	NULL			promoter	NULL	PFP-negative EL-4 cell line	0	NULL	NULL	NULL	gw60_immunity_17_4_437_s_194	12387738	(D) Chromatin immunoprecipitation analysis of MEF binding to PFP promoter in the PFP-positive CTLL-2 cell line but not the PFP-negative EL-4 cell line.	bind
13313	1	5033	6	NULL	NULL	NULL	NULL	Hip1R	GP		bind					cages		truncated			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_6_1209_s_78	11564758	(d) Clathrin LC restores Hip1R binding to truncated cages.	bind
13314	2	5033	6	NULL	NULL	NULL	NULL	Clathrin LC	GP		restores					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_6_1209_s_78	11564758	(d) Clathrin LC restores Hip1R binding to truncated cages.	bind
13413	1	5033	7	10	NULL	0	NULL	Hip1R	NULL		bind	NULL				cages	NULL	truncated			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_6_1209_s_78	11564758	(d) Clathrin LC restores Hip1R binding to truncated cages.	bind
13414	2	5033	7	NULL	NULL	0	NULL	Clathrin LC	NULL		restores	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_154_6_1209_s_78	11564758	(d) Clathrin LC restores Hip1R binding to truncated cages.	bind
13315	1	5034	6	NULL	NULL	NULL	NULL	CLOCK	GP		bind					mPer1	GP			E box at CT 06	NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_855_s_164	11779462	(D) CLOCK and BMAL1 are  bound to  mPer1 E box at CT  06 and 15.	bind
13316	2	5034	6	NULL	NULL	NULL	NULL	CLOCK	GP		bind					mPer1	GP			E box at CT 15	NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_855_s_164	11779462	(D) CLOCK and BMAL1 are  bound to  mPer1 E box at CT  06 and 15.	bind
13317	3	5034	6	NULL	NULL	NULL	NULL	BMAL1	GP		bind					mPer1	GP			E box at CT 06	NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_855_s_164	11779462	(D) CLOCK and BMAL1 are  bound to  mPer1 E box at CT  06 and 15.	bind
13318	4	5034	6	NULL	NULL	NULL	NULL	BMAL1	GP		bind					mPer1	GP			E box at CT 15	NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_855_s_164	11779462	(D) CLOCK and BMAL1 are  bound to  mPer1 E box at CT  06 and 15.	bind
13416	1	5034	7	NULL	NULL	0	NULL	CLOCK	NULL		bind	NULL				mPer1	NULL			E box at CT 06	NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_855_s_164	11779462	(D) CLOCK and BMAL1 are  bound to  mPer1 E box at CT  06 and 15.	bind
13419	2	5034	7	NULL	NULL	0	NULL	CLOCK	NULL		bind	NULL				 mPer1	NULL			E box at CT 15	NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_855_s_164	11779462	(D) CLOCK and BMAL1 are  bound to  mPer1 E box at CT  06 and 15.	bind
13420	3	5034	7	NULL	NULL	0	NULL	BMAL1	NULL		bind	NULL				mPer1	NULL			E box at CT 06	NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_855_s_164	11779462	(D) CLOCK and BMAL1 are  bound to  mPer1 E box at CT  06 and 15.	bind
13421	4	5034	7	NULL	NULL	0	NULL	BMAL1	NULL		bind	NULL				mPer1	NULL			E box at CT 15	NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_855_s_164	11779462	(D) CLOCK and BMAL1 are  bound to  mPer1 E box at CT  06 and 15.	bind
13319	1	5035	6	NULL	NULL	NULL	NULL	Tubulin	OrganismPart	soluble	bind					GST-CNP	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_170_4_661_s_71	16103231	(D) Comparative binding of soluble tubulin and preassembled MTs to GST-CNP.	bind
13320	2	5035	6	NULL	NULL	NULL	NULL	MTs	OrganismPart	preassembled	bind					GST-CNP	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_170_4_661_s_71	16103231	(D) Comparative binding of soluble tubulin and preassembled MTs to GST-CNP.	bind
13424	1	5035	7	NULL	NULL	0	NULL	tubulin	NULL	soluble	bind	NULL				GST-CNP	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_170_4_661_s_71	16103231	(D) Comparative binding of soluble tubulin and preassembled MTs to GST-CNP.	bind
13425	2	5035	7	NULL	NULL	0	NULL	MTs	NULL	preassembled	bind	NULL				GST-CNP	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_170_4_661_s_71	16103231	(D) Comparative binding of soluble tubulin and preassembled MTs to GST-CNP.	bind
13334	1	5039	6	NULL	NULL	NULL	NULL	myosin-Va	GP		bind					syntaxin-1A	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_161	16030255	(D) Competitive inhibition of myosin-Va binding to syntaxin-1A by syntaxin-1A [191-240].	bind
13335	2	5039	6	NULL	NULL	NULL	NULL	myosin-Va	GP		bind					syntaxin-1A	GP		191-240		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_161	16030255	(D) Competitive inhibition of myosin-Va binding to syntaxin-1A by syntaxin-1A [191-240].	bind
44703	3	5039	6	NULL	NULL	NULL	NULL	statement 2	Process		inhibit		competitively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_161	16030255	(D) Competitive inhibition of myosin-Va binding to syntaxin-1A by syntaxin-1A [191-240].	bind
13426	1	5039	7	NULL	NULL	0	NULL	myosin-Va	NULL		bind	NULL				syntaxin-1A	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_161	16030255	(D) Competitive inhibition of myosin-Va binding to syntaxin-1A by syntaxin-1A [191-240].	bind
13427	2	5039	7	NULL	NULL	0	NULL	myosin-Va	NULL		bind	NULL				syntaxin-1A 	NULL		191-240		NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_161	16030255	(D) Competitive inhibition of myosin-Va binding to syntaxin-1A by syntaxin-1A [191-240].	bind
13429	3	5039	7	NULL	NULL	0	NULL	statement 2	NULL		inhibits	NULL	competitively			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_161	16030255	(D) Competitive inhibition of myosin-Va binding to syntaxin-1A by syntaxin-1A [191-240].	bind
13491	1	5040	6	NULL	NULL	NULL	NULL	IAAP	GP		bind					Cdr1p-GFP	GP				NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_2_6_1361_s_197	14665469	(d) Concentration-dependent  inhibition of IAAP binding to Cdr1p-GFP by nystatin.	bind
13492	2	5040	6	NULL	NULL	NULL	NULL	nystatin	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_2_6_1361_s_197	14665469	(d) Concentration-dependent  inhibition of IAAP binding to Cdr1p-GFP by nystatin.	bind
13493	3	5040	6	NULL	NULL	NULL	NULL	statement 2	Process		is dependent on					concentration					NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_2_6_1361_s_197	14665469	(d) Concentration-dependent  inhibition of IAAP binding to Cdr1p-GFP by nystatin.	bind
13430	1	5040	7	NULL	NULL	0	NULL	IAAP	NULL		bind	NULL				Cdr1p-GFP	NULL				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_2_6_1361_s_197	14665469	(d) Concentration-dependent  inhibition of IAAP binding to Cdr1p-GFP by nystatin.	bind
13432	2	5040	7	NULL	NULL	0	NULL	nystatin	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_2_6_1361_s_197	14665469	(d) Concentration-dependent  inhibition of IAAP binding to Cdr1p-GFP by nystatin.	bind
13433	3	5040	7	NULL	NULL	0	NULL	statement 2	NULL		is dependent on	NULL				Concentration	NULL				NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_2_6_1361_s_197	14665469	(d) Concentration-dependent  inhibition of IAAP binding to Cdr1p-GFP by nystatin.	bind
13494	1	5043	6	NULL	NULL	NULL	NULL	Ccz1	GP		bind					vacuole	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_163_5_973_s_71	14662743	(D) Cooperative binding of Ccz1 and Mon1 to the vacuole.	bind
13495	2	5043	6	NULL	NULL	NULL	NULL	Mon1	GP		bind					vacuole	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_163_5_973_s_71	14662743	(D) Cooperative binding of Ccz1 and Mon1 to the vacuole.	bind
13496	3	5043	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_163_5_973_s_71	14662743	(D) Cooperative binding of Ccz1 and Mon1 to the vacuole.	bind
13434	1	5043	7	NULL	NULL	0	NULL	Ccz1	NULL		binds	NULL				vacuole	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_163_5_973_s_71	14662743	(D) Cooperative binding of Ccz1 and Mon1 to the vacuole.	bind
13436	2	5043	7	NULL	NULL	0	NULL	Mon1	NULL		binds	NULL				vacuole	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_163_5_973_s_71	14662743	(D) Cooperative binding of Ccz1 and Mon1 to the vacuole.	bind
13437	3	5043	7	NULL	NULL	0	NULL	statement 1	NULL		occurs in cooperation with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_163_5_973_s_71	14662743	(D) Cooperative binding of Ccz1 and Mon1 to the vacuole.	bind
13497	1	5044	6	NULL	NULL	NULL	NULL	NF-Y	GP		bind					AADC 	GP			neuronal promoter	NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_89_1_58_s_213	11311976	(D) Cooperative binding of NF-Y and the POU-domain of Brn-2 on AADC neuronal promoter.	bind
13498	2	5044	6	NULL	NULL	NULL	NULL	Brn-2	GP		bind			POU domain		AADC	GP			neuronal promoter	NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_89_1_58_s_213	11311976	(D) Cooperative binding of NF-Y and the POU-domain of Brn-2 on AADC neuronal promoter.	bind
13499	3	5044	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_89_1_58_s_213	11311976	(D) Cooperative binding of NF-Y and the POU-domain of Brn-2 on AADC neuronal promoter.	bind
13439	1	5044	7	10	NULL	0	NULL	NF-Y	NULL		binds	NULL				AADC	NULL			 neuronal promoter	NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_89_1_58_s_213	11311976	(D) Cooperative binding of NF-Y and the POU-domain of Brn-2 on AADC neuronal promoter.	bind
13440	2	5044	7	10	NULL	0	NULL	Brn-2	NULL		binds	NULL		POU		AADC	NULL			neuronal promoter	NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_89_1_58_s_213	11311976	(D) Cooperative binding of NF-Y and the POU-domain of Brn-2 on AADC neuronal promoter.	bind
13441	3	5044	7	NULL	NULL	0	NULL	statement 1	NULL		occurs in cooperation with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_brainresmolbrainres_89_1_58_s_213	11311976	(D) Cooperative binding of NF-Y and the POU-domain of Brn-2 on AADC neuronal promoter.	bind
13500	1	5046	6	NULL	NULL	NULL	NULL	CPI-17	GP		bind		directly			CKI	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_1_39_s_143	15003508	(D) CPI-17 directly binds to CKI.	bind
13442	1	5046	7	NULL	NULL	0	NULL	CPI-17	NULL		binds	NULL	directly			CKI	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_1_39_s_143	15003508	(D) CPI-17 directly binds to CKI.	bind
13501	1	5047	6	NULL	NULL	NULL	NULL	CUGBP1	GP		bind					p21 mRNA	NucleicAcid			GCN repeats;;5' region	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_20_6927_s_254	11564876	(D) CUGBP1 binds to GCN repeats with the 5' region of p21 mRNA.	bind
13443	1	5047	7	10	NULL	0	NULL	CUGBP1	NULL		binds	NULL				p21 mRNA	NULL			GCN repeats;;5' region 	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_20_6927_s_254	11564876	(D) CUGBP1 binds to GCN repeats with the 5' region of p21 mRNA.	bind
13502	1	5048	6	NULL	NULL	NULL	NULL	CUGBP2	GP		bind					COX-2	GP			first 60 nt of 3' UTR	NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_1_113_s_191	12535526	(D) CUGBP2 and hnRNP A1 bind cooperatively to the first 60 nt of COX-2 3 UTR.	bind
13503	2	5048	6	NULL	NULL	NULL	NULL	hnRNP A1	GP		bind					COX-2	GP			first 60 nt of 3' UTR	NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_1_113_s_191	12535526	(D) CUGBP2 and hnRNP A1 bind cooperatively to the first 60 nt of COX-2 3 UTR.	bind
13504	3	5048	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_1_113_s_191	12535526	(D) CUGBP2 and hnRNP A1 bind cooperatively to the first 60 nt of COX-2 3 UTR.	bind
13444	1	5048	7	NULL	NULL	0	NULL	CUGBP2	NULL		bind	NULL				COX-2	NULL			first 60 nt of 3 UTR	NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_1_113_s_191	12535526	(D) CUGBP2 and hnRNP A1 bind cooperatively to the first 60 nt of COX-2 3 UTR.	bind
13445	2	5048	7	NULL	NULL	0	NULL	 hnRNP A1	NULL		bind	NULL				COX-2	NULL			first 60 nt of 3 UTR	NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_1_113_s_191	12535526	(D) CUGBP2 and hnRNP A1 bind cooperatively to the first 60 nt of COX-2 3 UTR.	bind
13446	3	5048	7	NULL	NULL	0	NULL	statement 1 	NULL		occurs in cooperation with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_113_s_191	12535526	(D) CUGBP2 and hnRNP A1 bind cooperatively to the first 60 nt of COX-2 3 UTR.	bind
13505	1	5049	6	NULL	NULL	NULL	NULL	Cyclin B chimeras	GP		bind					CDK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_945_s_197	11238451	(D) Cyclin B chimeras bind and activate CDK1 to a similar extent as wild-type cyclins.	bind
13506	2	5049	6	NULL	NULL	NULL	NULL	Cyclin B chimeras	GP		activate					CDK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_945_s_197	11238451	(D) Cyclin B chimeras bind and activate CDK1 to a similar extent as wild-type cyclins.	bind
13507	3	5049	6	NULL	NULL	NULL	NULL	cyclins	GP	wild type	bind					CDK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_945_s_197	11238451	(D) Cyclin B chimeras bind and activate CDK1 to a similar extent as wild-type cyclins.	bind
13508	4	5049	6	NULL	NULL	NULL	NULL	cyclins	GP	wild type	activate					CDK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_945_s_197	11238451	(D) Cyclin B chimeras bind and activate CDK1 to a similar extent as wild-type cyclins.	bind
44714	5	5049	6	NULL	NULL	NULL	NULL	statement 1	Process		is similar to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_945_s_197	11238451	(D) Cyclin B chimeras bind and activate CDK1 to a similar extent as wild-type cyclins.	bind
44715	6	5049	6	NULL	NULL	NULL	NULL	statement 2	Process		is similar to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_945_s_197	11238451	(D) Cyclin B chimeras bind and activate CDK1 to a similar extent as wild-type cyclins.	bind
13459	1	5049	7	NULL	NULL	0	NULL	Cyclin B chimera	NULL		bind	NULL				CDK1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_945_s_197	11238451	(D) Cyclin B chimeras bind and activate CDK1 to a similar extent as wild-type cyclins.	bind
13460	2	5049	7	NULL	NULL	0	NULL	Cyclin B chimera	NULL		activate	NULL				CDK1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_945_s_197	11238451	(D) Cyclin B chimeras bind and activate CDK1 to a similar extent as wild-type cyclins.	bind
13462	3	5049	7	NULL	NULL	0	NULL	cyclins	NULL	wild-type	bind	NULL				CDK1	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_152_5_945_s_197	11238451	(D) Cyclin B chimeras bind and activate CDK1 to a similar extent as wild-type cyclins.	bind
13464	5	5049	7	NULL	NULL	0	NULL	statement 1	NULL		occurs to a similar extent as	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_945_s_197	11238451	(D) Cyclin B chimeras bind and activate CDK1 to a similar extent as wild-type cyclins.	bind
17357	4	5049	7	NULL	NULL	0	NULL	cyclins	NULL	wild-type	activate	NULL				CDK1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_945_s_197	11238451	(D) Cyclin B chimeras bind and activate CDK1 to a similar extent as wild-type cyclins.	bind
44721	6	5049	7	NULL	NULL	0	NULL	statement 2	NULL		occurs to a similar extent as	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_152_5_945_s_197	11238451	(D) Cyclin B chimeras bind and activate CDK1 to a similar extent as wild-type cyclins.	bind
13509	1	5050	6	NULL	NULL	NULL	NULL	DDB1	GP		bind		directly			DDB2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_113_3_357_s_61	12732143	(D) DDB1 directly binds not only to DDB2, but also to CSA.	bind
13510	2	5050	6	NULL	NULL	NULL	NULL	DDB1	GP		bind		directly			CSA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_113_3_357_s_61	12732143	(D) DDB1 directly binds not only to DDB2, but also to CSA.	bind
13465	1	5050	7	NULL	NULL	0	NULL	DDB1	NULL		binds	NULL	directly			DDB2	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_113_3_357_s_61	12732143	(D) DDB1 directly binds not only to DDB2, but also to CSA.	bind
13466	2	5050	7	NULL	NULL	0	NULL	DDB1	NULL		binds	NULL	directly			CSA	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_113_3_357_s_61	12732143	(D) DDB1 directly binds not only to DDB2, but also to CSA.	bind
13511	1	5051	6	NULL	NULL	NULL	NULL	FoxM1 protein	GP		bind					Skp2	GP	endogenous		promoter	NULL	U2OS cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_24_10875_s_386	16314512	(D) Depletion of FoxM1 in U2OS cells by siFoxM1 #2 transfection  inhibits binding of FoxM1 protein to the endogenous Skp2 or Cks1 promoter regions.	bind
13512	2	5051	6	NULL	NULL	NULL	NULL	FoxM1 protein	GP		bind					Cks1	GP	endogenous		promoter	NULL	U2OS cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_24_10875_s_386	16314512	(D) Depletion of FoxM1 in U2OS cells by siFoxM1 #2 transfection  inhibits binding of FoxM1 protein to the endogenous Skp2 or Cks1 promoter regions.	bind
13513	3	5051	6	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_24_10875_s_386	16314512	(D) Depletion of FoxM1 in U2OS cells by siFoxM1 #2 transfection  inhibits binding of FoxM1 protein to the endogenous Skp2 or Cks1 promoter regions.	bind
13514	4	5051	6	NULL	NULL	NULL	NULL	FoxM1 protein	GP	depletion of 	inhibits					statement 1	Process				NULL	U2OS cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_24_10875_s_386	16314512	(D) Depletion of FoxM1 in U2OS cells by siFoxM1 #2 transfection  inhibits binding of FoxM1 protein to the endogenous Skp2 or Cks1 promoter regions.	bind
13515	5	5051	6	NULL	NULL	NULL	NULL	FoxM1 protein	GP	depletion of	inhibits					statement 2	Process				NULL	U2OS cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_24_10875_s_386	16314512	(D) Depletion of FoxM1 in U2OS cells by siFoxM1 #2 transfection  inhibits binding of FoxM1 protein to the endogenous Skp2 or Cks1 promoter regions.	bind
13467	1	5051	7	NULL	NULL	0	NULL	FoxM1	NULL		bind	NULL				Skp2	NULL	endogenous		promoter	NULL	U2OS cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_24_10875_s_386	16314512	(D) Depletion of FoxM1 in U2OS cells by siFoxM1 #2 transfection  inhibits binding of FoxM1 protein to the endogenous Skp2 or Cks1 promoter regions.	bind
13468	2	5051	7	NULL	NULL	0	NULL	FoxM1	NULL		bind	NULL				Cks1	NULL	endogenous		promoter	NULL	U2OS cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_24_10875_s_386	16314512	(D) Depletion of FoxM1 in U2OS cells by siFoxM1 #2 transfection  inhibits binding of FoxM1 protein to the endogenous Skp2 or Cks1 promoter regions.	bind
13469	3	5051	7	10	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_24_10875_s_386	16314512	(D) Depletion of FoxM1 in U2OS cells by siFoxM1 #2 transfection  inhibits binding of FoxM1 protein to the endogenous Skp2 or Cks1 promoter regions.	bind
13470	4	5051	7	10	NULL	0	NULL	FoxM1	NULL	depletion of	inhibits	NULL				statement 1	NULL				NULL	U2OS cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_24_10875_s_386	16314512	(D) Depletion of FoxM1 in U2OS cells by siFoxM1 #2 transfection  inhibits binding of FoxM1 protein to the endogenous Skp2 or Cks1 promoter regions.	bind
13471	5	5051	7	10	NULL	0	NULL	FoxM1	NULL	depletion of	inhibits	NULL				statement 2	NULL				NULL	U2OS cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_24_10875_s_386	16314512	(D) Depletion of FoxM1 in U2OS cells by siFoxM1 #2 transfection  inhibits binding of FoxM1 protein to the endogenous Skp2 or Cks1 promoter regions.	bind
13516	1	5053	6	NULL	NULL	NULL	NULL	TIP60	GP		bind		differentially			p21 gene	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4006_s_234	16705155	(D) Differential binding of TIP60 and GAS41 to  p21 and  p14 ARF gene promoters.	bind
13517	2	5053	6	NULL	NULL	NULL	NULL	GAS41	GP		bind		differentially			p21 gene	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4006_s_234	16705155	(D) Differential binding of TIP60 and GAS41 to  p21 and  p14 ARF gene promoters.	bind
13518	3	5053	6	NULL	NULL	NULL	NULL	TIP60	GP		bind		differentially			p14 ARF gene	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4006_s_234	16705155	(D) Differential binding of TIP60 and GAS41 to  p21 and  p14 ARF gene promoters.	bind
13519	4	5053	6	NULL	NULL	NULL	NULL	GAS41	GP		bind		differentially			p14 ARF gene	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4006_s_234	16705155	(D) Differential binding of TIP60 and GAS41 to  p21 and  p14 ARF gene promoters.	bind
13472	1	5053	7	10	NULL	0	NULL	TIP60 	NULL		binds	NULL	differentially			p21 gene	NULL			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4006_s_234	16705155	(D) Differential binding of TIP60 and GAS41 to  p21 and  p14 ARF gene promoters.	bind
13473	2	5053	7	10	NULL	0	NULL	TIP60 	NULL		binds	NULL	differentially			p14 ARF gene	NULL			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4006_s_234	16705155	(D) Differential binding of TIP60 and GAS41 to  p21 and  p14 ARF gene promoters.	bind
13474	3	5053	7	10	NULL	0	NULL	GAS41	NULL		binds	NULL	differentially			p21 gene	NULL			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4006_s_234	16705155	(D) Differential binding of TIP60 and GAS41 to  p21 and  p14 ARF gene promoters.	bind
13475	4	5053	7	10	NULL	0	NULL	GAS41	NULL		binds	NULL	differentially			p14 ARF gene	NULL			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4006_s_234	16705155	(D) Differential binding of TIP60 and GAS41 to  p21 and  p14 ARF gene promoters.	bind
13520	1	5054	6	NULL	NULL	NULL	NULL	GCNF	GP		bind		directly			Nanog gene	GP	endogenous		DR0 element	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8507_s_254	16166633	(D) Direct binding of GCNF to the endogenous   Nanog gene DR0 elements was demonstrated by ChIP assay with GCNF antibodies.	bind
13476	1	5054	7	10	NULL	0	NULL	GCNF	NULL		binds	NULL	directly			Nanog gene	NULL	endogenous		DR0 element	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8507_s_254	16166633	(D) Direct binding of GCNF to the endogenous   Nanog gene DR0 elements was demonstrated by ChIP assay with GCNF antibodies.	bind
13521	1	5055	6	NULL	NULL	NULL	NULL	His6-Ipl1	GP		bind		directly			GST-Sli15	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_7_1381_s_298	10385519	(D) Direct binding of His6-Ipl1  to GST-Sli15.	bind
13477	1	5055	7	NULL	NULL	0	NULL	His6-Ipl1	NULL		binds	NULL	directly			GST-Sli15	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_7_1381_s_298	10385519	(D) Direct binding of His6-Ipl1  to GST-Sli15.	bind
13522	1	5056	6	NULL	NULL	NULL	NULL	Dkk-1	GP		bind					LRP5/6	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_278	11448771	(d) Dkk-1 binds to LRP5/6 and prevents Fz-LRP5/6 complex formation but does not affect the Wnt-Fz interaction.	bind
13524	3	5056	6	NULL	NULL	NULL	NULL	statement 1	Process		prevents					Fz-LRP5/6 complex	GP	formation of			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_278	11448771	(d) Dkk-1 binds to LRP5/6 and prevents Fz-LRP5/6 complex formation but does not affect the Wnt-Fz interaction.	bind
13526	5	5056	6	NULL	NULL	NULL	NULL	statement 1	Process		has no effect on					Wnt-Fz	GP	interaction of			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_278	11448771	(d) Dkk-1 binds to LRP5/6 and prevents Fz-LRP5/6 complex formation but does not affect the Wnt-Fz interaction.	bind
13478	1	5056	7	NULL	NULL	0	NULL	Dkk-1	NULL		binds	NULL				LRP5/6	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_278	11448771	(d) Dkk-1 binds to LRP5/6 and prevents Fz-LRP5/6 complex formation but does not affect the Wnt-Fz interaction.	bind
13479	2	5056	7	NULL	NULL	0	NULL	statement 1	NULL		prevents	NULL				Fz-LRP5/6 complex	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_278	11448771	(d) Dkk-1 binds to LRP5/6 and prevents Fz-LRP5/6 complex formation but does not affect the Wnt-Fz interaction.	bind
13481	4	5056	7	10	NULL	0	NULL	statement 1	NULL		does not affect	NULL				Wnt-Fz	NULL	interaction of			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_278	11448771	(d) Dkk-1 binds to LRP5/6 and prevents Fz-LRP5/6 complex formation but does not affect the Wnt-Fz interaction.	bind
13527	1	5057	6	NULL	NULL	NULL	NULL	Dock	GP		bind			SH3 domain		Dscam	GP				NULL	yeast 	NULL	NULL	NULL	NULL	gw60_cell_101_6_671_s_115	10892653	(D) Dock  SH3 domains bind Dscam in yeast.	bind
13482	1	5057	7	10	NULL	0	NULL	Dock	NULL		bind	NULL		SH3 domain		Dscam	NULL				NULL	yeast	NULL	NULL	NULL	NULL	gw60_cell_101_6_671_s_115	10892653	(D) Dock  SH3 domains bind Dscam in yeast.	bind
13528	1	5058	6	NULL	NULL	NULL	NULL	E. coli SE5000(pCS267)	Organism	Psa-fimbriated	bind					A549 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_74_10_5636_s_128	16988239	(D) Dose-dependent  inhibition of Psa-fimbriated  E. coli SE5000(pCS267) binding to A549 cells using rabbit-specific anti-Psa (filled circles)  or preimmune (empty circles) antiserum as inhibitors.	bind
13529	2	5058	6	NULL	NULL	NULL	NULL	rabbit-specific anti-Psa	GP		inhibits		dose dependently			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_74_10_5636_s_128	16988239	(D) Dose-dependent  inhibition of Psa-fimbriated  E. coli SE5000(pCS267) binding to A549 cells using rabbit-specific anti-Psa (filled circles)  or preimmune (empty circles) antiserum as inhibitors.	bind
13530	3	5058	6	NULL	NULL	NULL	NULL	preimmune antiserum			inhibits		dose dependently			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_74_10_5636_s_128	16988239	(D) Dose-dependent  inhibition of Psa-fimbriated  E. coli SE5000(pCS267) binding to A549 cells using rabbit-specific anti-Psa (filled circles)  or preimmune (empty circles) antiserum as inhibitors.	bind
13483	1	5058	7	10	NULL	0	NULL	E. coli SE5000(pCS267)	NULL	Psa-fimbriated	bind	NULL				A549 cells 	NULL				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_74_10_5636_s_128	16988239	(D) Dose-dependent  inhibition of Psa-fimbriated  E. coli SE5000(pCS267) binding to A549 cells using rabbit-specific anti-Psa (filled circles)  or preimmune (empty circles) antiserum as inhibitors.	bind
13484	2	5058	7	NULL	NULL	0	NULL	rabbit-specific anti-Psa	NULL		inhibits	NULL	dose-dependently			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_74_10_5636_s_128	16988239	(D) Dose-dependent  inhibition of Psa-fimbriated  E. coli SE5000(pCS267) binding to A549 cells using rabbit-specific anti-Psa (filled circles)  or preimmune (empty circles) antiserum as inhibitors.	bind
13485	3	5058	7	NULL	NULL	0	NULL	preimmune antiserum	NULL		inhibits	NULL	dose-dependently			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_74_10_5636_s_128	16988239	(D) Dose-dependent  inhibition of Psa-fimbriated  E. coli SE5000(pCS267) binding to A549 cells using rabbit-specific anti-Psa (filled circles)  or preimmune (empty circles) antiserum as inhibitors.	bind
13531	1	5059	6	NULL	NULL	NULL	NULL	Hsf4b	GP		bind									HSE	NULL	H1299 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_8_3282_s_206	16581800	(D) DUSP26 affects  Hsf4b binding to HSE. H1299 cells were cotransfected with Flag-Hsf4b and increasing  amounts of HA-DUSP26 (same samples as in panel A, lanes 1 to 4).	bind
13532	2	5059	6	NULL	NULL	NULL	NULL	DUSP26	GP		affects					statement 1	Process				NULL	H1299 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_8_3282_s_206	16581800	(D) DUSP26 affects  Hsf4b binding to HSE. H1299 cells were cotransfected with Flag-Hsf4b and increasing  amounts of HA-DUSP26 (same samples as in panel A, lanes 1 to 4).	bind
13486	1	5059	7	NULL	NULL	0	NULL	Flag-Hsf4b	NULL		binds	NULL					NULL			HSE	NULL	H1299 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_8_3282_s_206	16581800	(D) DUSP26 affects  Hsf4b binding to HSE. H1299 cells were cotransfected with Flag-Hsf4b and increasing  amounts of HA-DUSP26 (same samples as in panel A, lanes 1 to 4).	bind
13487	2	5059	7	NULL	NULL	0	NULL	HA-DUSP26	NULL		affects	NULL				statement 1	NULL				NULL	H1299 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_8_3282_s_206	16581800	(D) DUSP26 affects  Hsf4b binding to HSE. H1299 cells were cotransfected with Flag-Hsf4b and increasing  amounts of HA-DUSP26 (same samples as in panel A, lanes 1 to 4).	bind
13533	1	5060	6	NULL	NULL	NULL	NULL	GR	GP		bind					MMTV	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_10_3255_s_79	11971959	(D) Effect of HMG-1 on binding of GR to MMTV promoter.	bind
13488	1	5060	7	NULL	NULL	0	NULL	GR	NULL		bind	NULL				MMTV	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_10_3255_s_79	11971959	(D) Effect of HMG-1 on binding of GR to MMTV promoter.	bind
13534	1	5061	6	NULL	NULL	NULL	NULL	MAb 24c5	GP		bind					M. tuberculosis Erdman day-20 7H9 medium					NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_147	11953397	(D) Effects of proteinase K on binding of MAb 24c5 to  M. tuberculosis Erdman day-20 7H9 medium.	bind
13489	1	5061	7	NULL	NULL	0	NULL	MAb 24c5	NULL		bind	NULL				M. tuberculosis Erdman day-20 7H9 medium	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_5_2566_s_147	11953397	(D) Effects of proteinase K on binding of MAb 24c5 to  M. tuberculosis Erdman day-20 7H9 medium.	bind
13535	1	5062	6	NULL	NULL	NULL	NULL	GAL4-FAST2	GP		bind					n2 oligonucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_1_35_s_74	10678167	(D) EMSA analysis of the binding of a GAL4-FAST2 fusion protein to the oligonucleotide  n2.	bind
44670	2	5062	6	NULL	NULL	NULL	NULL	GAL4-FAST2	GP		is a type of					fusion protein					NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_1_35_s_74	10678167	(D) EMSA analysis of the binding of a GAL4-FAST2 fusion protein to the oligonucleotide  n2.	bind
13490	1	5062	7	NULL	NULL	0	NULL	GAL4-FAST2	NULL		binds	NULL				oligonucleotide n2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_5_1_35_s_74	10678167	(D) EMSA analysis of the binding of a GAL4-FAST2 fusion protein to the oligonucleotide  n2.	bind
44671	2	5062	7	10	NULL	0	NULL	GAL4-FAST2	NULL		is a type of	NULL				fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_5_1_35_s_74	10678167	(D) EMSA analysis of the binding of a GAL4-FAST2 fusion protein to the oligonucleotide  n2.	bind
13536	1	5063	6	NULL	NULL	NULL	NULL	Sp1	GP		bind					DNA	NucleicAcid				NULL	kidney nuclear extracts	NULL	NULL	NULL	NULL	gw70_devbiol_267_2_505_s_227	15013809	(D) EMSA analysis with kidney (K) and liver (L) nuclear extracts shows  equivalent Sp1 and Sp3 DNA binding activity.	bind
13537	2	5063	6	NULL	NULL	NULL	NULL	Sp1	GP		bind					DNA	NucleicAcid				NULL	liver nuclear extracts	NULL	NULL	NULL	NULL	gw70_devbiol_267_2_505_s_227	15013809	(D) EMSA analysis with kidney (K) and liver (L) nuclear extracts shows  equivalent Sp1 and Sp3 DNA binding activity.	bind
13538	3	5063	6	NULL	NULL	NULL	NULL	Sp3	GP		bind					DNA	NucleicAcid				NULL	kidney nuclear extracts	NULL	NULL	NULL	NULL	gw70_devbiol_267_2_505_s_227	15013809	(D) EMSA analysis with kidney (K) and liver (L) nuclear extracts shows  equivalent Sp1 and Sp3 DNA binding activity.	bind
13539	4	5063	6	NULL	NULL	NULL	NULL	sp3	GP		bind					DNA	NucleicAcid				NULL	liver nuclear extracts	NULL	NULL	NULL	NULL	gw70_devbiol_267_2_505_s_227	15013809	(D) EMSA analysis with kidney (K) and liver (L) nuclear extracts shows  equivalent Sp1 and Sp3 DNA binding activity.	bind
17715	5	5063	6	NULL	NULL	0	NULL	K	NULL		is	NULL				Kidney	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_267_2_505_s_227	15013809	(D) EMSA analysis with kidney (K) and liver (L) nuclear extracts shows  equivalent Sp1 and Sp3 DNA binding activity.	bind
17716	6	5063	6	NULL	NULL	0	NULL	L	NULL		is	NULL				liver	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_267_2_505_s_227	15013809	(D) EMSA analysis with kidney (K) and liver (L) nuclear extracts shows  equivalent Sp1 and Sp3 DNA binding activity.	bind
13614	1	5063	7	10	NULL	0	NULL	Sp1 	NULL		bind	NULL				DNA	NULL				NULL	Kidney nuclear extract	NULL	NULL	NULL	NULL	gw70_devbiol_267_2_505_s_227	15013809	(D) EMSA analysis with kidney (K) and liver (L) nuclear extracts shows  equivalent Sp1 and Sp3 DNA binding activity.	bind
13615	2	5063	7	NULL	NULL	0	NULL	Sp1	NULL		bind	NULL				DNA	NULL				NULL	Liver nuclear extract	0	NULL	NULL	NULL	gw70_devbiol_267_2_505_s_227	15013809	(D) EMSA analysis with kidney (K) and liver (L) nuclear extracts shows  equivalent Sp1 and Sp3 DNA binding activity.	bind
13616	3	5063	7	10	NULL	0	NULL	 Sp3	NULL		bind	NULL				DNA	NULL				NULL	Kidney nuclear extract	NULL	NULL	NULL	NULL	gw70_devbiol_267_2_505_s_227	15013809	(D) EMSA analysis with kidney (K) and liver (L) nuclear extracts shows  equivalent Sp1 and Sp3 DNA binding activity.	bind
13617	4	5063	7	NULL	NULL	0	NULL	Sp3	NULL		bind	NULL				DNA	NULL				NULL	Liver nuclear extract	0	NULL	NULL	NULL	gw70_devbiol_267_2_505_s_227	15013809	(D) EMSA analysis with kidney (K) and liver (L) nuclear extracts shows  equivalent Sp1 and Sp3 DNA binding activity.	bind
13618	5	5063	7	NULL	NULL	0	NULL	Kidney	NULL		is	NULL				K	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_267_2_505_s_227	15013809	(D) EMSA analysis with kidney (K) and liver (L) nuclear extracts shows  equivalent Sp1 and Sp3 DNA binding activity.	bind
13619	6	5063	7	NULL	NULL	0	NULL	Liver	NULL		is	NULL				L	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_267_2_505_s_227	15013809	(D) EMSA analysis with kidney (K) and liver (L) nuclear extracts shows  equivalent Sp1 and Sp3 DNA binding activity.	bind
13540	1	5064	6	NULL	NULL	NULL	NULL	Runx2	GP	endogenous	bind					beta-casein	GP			Runx2-binding site of promoter	NULL	HC11 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3182_s_108	15798204	(D) EMSA demonstrating  that endogenous Runx2 from HC11 cells binds to the Runx2-binding site in the beta-casein  promoter.	bind
13620	1	5064	7	10	NULL	0	NULL	Runx2	NULL	endogenous	binds	NULL				beta-casein	NULL			Runx2-binding site in the promoter of 	NULL	 HC11 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3182_s_108	15798204	(D) EMSA demonstrating  that endogenous Runx2 from HC11 cells binds to the Runx2-binding site in the beta-casein  promoter.	bind
13541	1	5066	6	NULL	NULL	NULL	NULL	GST-HoxB5	GP	recombinant	bind		specifically			HBE					NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_16_5680_s_184	12897140	(D) EMSA with recombinant GST-HoxB5 (or GST alone) indicating specific  binding to the HBE that is competed away by excess specific (+) competitor but not  by a mutant sequence (NS).	bind
13622	1	5066	7	NULL	NULL	0	NULL	GST-HoxB5	NULL	recombinant	binds	NULL	specifically			HBE	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_16_5680_s_184	12897140	(D) EMSA with recombinant GST-HoxB5 (or GST alone) indicating specific  binding to the HBE that is competed away by excess specific (+) competitor but not  by a mutant sequence (NS).	bind
13542	1	5068	6	NULL	NULL	NULL	NULL	calsyntenin-1	GP		bind					KLC1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_8_3651_s_120	16760430	(D) Estimation of the  apparent binding affinity of calsyntenin-1 to KLC1.	bind
13625	1	5068	7	NULL	NULL	0	NULL	calsyntenin-1	NULL		bind	NULL				KLC1	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_8_3651_s_120	16760430	(D) Estimation of the  apparent binding affinity of calsyntenin-1 to KLC1.	bind
13543	1	5070	6	NULL	NULL	NULL	NULL	FH	GP		bind					Fba	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_71_12_7119_s_166	14638802	(D) FH  binding to immobilized Fba.	bind
13630	1	5070	7	NULL	NULL	0	NULL	FH	NULL		binds	NULL				Fba	NULL	immobilized			NULL		0	NULL	NULL	NULL	gw70_infectimmun_71_12_7119_s_166	14638802	(D) FH  binding to immobilized Fba.	bind
13586	1	5071	6	NULL	NULL	NULL	NULL	NrbI protein	GP		induces					Filopodia	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_5_2349_s_137	15743906	(D) Filopodia induced by NrbI and Spino proteins unable to bind PP1 because  of the F-to-A substitutions within the PP1-binding motif were compared with control  GFP-expressing cells as described above.	bind
13587	2	5071	6	NULL	NULL	NULL	NULL	spino proteins	GP		induce					Filopodia	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_5_2349_s_137	15743906	(D) Filopodia induced by NrbI and Spino proteins unable to bind PP1 because  of the F-to-A substitutions within the PP1-binding motif were compared with control  GFP-expressing cells as described above.	bind
13588	3	5071	6	NULL	NULL	NULL	NULL	statement 6	Process		does not bind					PP1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_5_2349_s_137	15743906	(D) Filopodia induced by NrbI and Spino proteins unable to bind PP1 because  of the F-to-A substitutions within the PP1-binding motif were compared with control  GFP-expressing cells as described above.	bind
13773	4	5071	6	NULL	NULL	NULL	NULL	statement 1	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_5_2349_s_137	15743906	(D) Filopodia induced by NrbI and Spino proteins unable to bind PP1 because  of the F-to-A substitutions within the PP1-binding motif were compared with control  GFP-expressing cells as described above.	bind
13774	5	5071	6	NULL	NULL	NULL	NULL	statement 2	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_5_2349_s_137	15743906	(D) Filopodia induced by NrbI and Spino proteins unable to bind PP1 because  of the F-to-A substitutions within the PP1-binding motif were compared with control  GFP-expressing cells as described above.	bind
53050	6	5071	6	NULL	NULL	NULL	NULL	Filopodia	OrganismPart		is substituted to			F within PP1-binding motif		Filopodia	OrganismPart		A within PP1-binding motif		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_5_2349_s_137	15743906	(D) Filopodia induced by NrbI and Spino proteins unable to bind PP1 because  of the F-to-A substitutions within the PP1-binding motif were compared with control  GFP-expressing cells as described above.	bind
13637	1	5071	7	NULL	NULL	0	NULL	NrbI protein	NULL		induce	NULL				Filopodia	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_5_2349_s_137	15743906	(D) Filopodia induced by NrbI and Spino proteins unable to bind PP1 because  of the F-to-A substitutions within the PP1-binding motif were compared with control  GFP-expressing cells as described above.	bind
13639	2	5071	7	NULL	NULL	0	NULL	Spino protein	NULL		induce	NULL				Filopodia	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_5_2349_s_137	15743906	(D) Filopodia induced by NrbI and Spino proteins unable to bind PP1 because  of the F-to-A substitutions within the PP1-binding motif were compared with control  GFP-expressing cells as described above.	bind
13653	3	5071	7	10	NULL	0	NULL	statement 6	NULL		does not bind	NULL				PP1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_5_2349_s_137	15743906	(D) Filopodia induced by NrbI and Spino proteins unable to bind PP1 because  of the F-to-A substitutions within the PP1-binding motif were compared with control  GFP-expressing cells as described above.	bind
13654	4	5071	7	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_5_2349_s_137	15743906	(D) Filopodia induced by NrbI and Spino proteins unable to bind PP1 because  of the F-to-A substitutions within the PP1-binding motif were compared with control  GFP-expressing cells as described above.	bind
13789	5	5071	7	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_5_2349_s_137	15743906	(D) Filopodia induced by NrbI and Spino proteins unable to bind PP1 because  of the F-to-A substitutions within the PP1-binding motif were compared with control  GFP-expressing cells as described above.	bind
53051	6	5071	7	10	NULL	0	NULL	Filopodia	NULL		is substituted to	NULL		F within PP1-binding motif		Filopodia	NULL		A within PP1-binding motif		NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_5_2349_s_137	15743906	(D) Filopodia induced by NrbI and Spino proteins unable to bind PP1 because  of the F-to-A substitutions within the PP1-binding motif were compared with control  GFP-expressing cells as described above.	bind
13544	1	5072	6	NULL	NULL	NULL	NULL	O2	Chemical		bind					hemes	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_68_3_453_s_89	15353565	(D) FixL acts  as a homodimer that is inactive when O2 is bound to the hemes.	bind
13545	2	5072	6	NULL	NULL	NULL	NULL	FixL	GP		acts as a					homodimer	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_68_3_453_s_89	15353565	(D) FixL acts  as a homodimer that is inactive when O2 is bound to the hemes.	bind
13546	3	5072	6	NULL	NULL	NULL	NULL	statement 1	Process		inactivates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_68_3_453_s_89	15353565	(D) FixL acts  as a homodimer that is inactive when O2 is bound to the hemes.	bind
13655	1	5072	7	NULL	NULL	0	NULL	O2	NULL		binds	NULL				heme	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_68_3_453_s_89	15353565	(D) FixL acts  as a homodimer that is inactive when O2 is bound to the hemes.	bind
13656	2	5072	7	NULL	NULL	0	NULL	FixL	NULL		acts as a 	NULL				homodimer	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_68_3_453_s_89	15353565	(D) FixL acts  as a homodimer that is inactive when O2 is bound to the hemes.	bind
13657	3	5072	7	NULL	NULL	0	NULL	statement 1	NULL		inactivates	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_68_3_453_s_89	15353565	(D) FixL acts  as a homodimer that is inactive when O2 is bound to the hemes.	bind
13547	1	5074	6	NULL	NULL	NULL	NULL	FXR	GP		bind					GRIP1	GP		NID region		NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_4_1093_s_58	12718893	(D) FXR binding to different NID regions of GRIP1 in the presence of CDCA.	bind
13548	2	5074	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs in presence of					CDCA	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_4_1093_s_58	12718893	(D) FXR binding to different NID regions of GRIP1 in the presence of CDCA.	bind
13660	1	5074	7	10	NULL	0	NULL	FXR	NULL		bind	NULL				GRIP1	NULL		NID region		NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_4_1093_s_58	12718893	(D) FXR binding to different NID regions of GRIP1 in the presence of CDCA.	bind
13661	2	5074	7	NULL	NULL	0	NULL	statement 1	NULL		occurs in the presence of	NULL				CDCA	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_11_4_1093_s_58	12718893	(D) FXR binding to different NID regions of GRIP1 in the presence of CDCA.	bind
13589	1	5075	6	NULL	NULL	NULL	NULL	L1	GP		bind					NP-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_23_6348_s_129	12456642	(d) G121S, a mutation that destroys homophilic binding, does not affect L1 binding to NP-1 or alter the ability of the chimera to induce the switch.	bind
13590	2	5075	6	NULL	NULL	0	NULL		NULL	mutant	destroys	NULL		G121S		homophilic binding	NULL				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_23_6348_s_129	12456642	(d) G121S, a mutation that destroys homophilic binding, does not affect L1 binding to NP-1 or alter the ability of the chimera to induce the switch.	bind
13591	3	5075	6	NULL	NULL	0	NULL		NULL	mutant	does not affect	NULL		G121S		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_21_23_6348_s_129	12456642	(d) G121S, a mutation that destroys homophilic binding, does not affect L1 binding to NP-1 or alter the ability of the chimera to induce the switch.	bind
13592	4	5075	6	NULL	NULL	0	NULL	chimera	NULL		induce	NULL				switch	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_21_23_6348_s_129	12456642	(d) G121S, a mutation that destroys homophilic binding, does not affect L1 binding to NP-1 or alter the ability of the chimera to induce the switch.	bind
13593	5	5075	6	NULL	NULL	0	NULL		NULL	mutant	does not alter	NULL		G121S		statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_21_23_6348_s_129	12456642	(d) G121S, a mutation that destroys homophilic binding, does not affect L1 binding to NP-1 or alter the ability of the chimera to induce the switch.	bind
13662	1	5075	7	10	NULL	0	NULL		NULL	mutant	destroys	NULL		G121S		homophilic binding	NULL				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_23_6348_s_129	12456642	(d) G121S, a mutation that destroys homophilic binding, does not affect L1 binding to NP-1 or alter the ability of the chimera to induce the switch.	bind
13663	2	5075	7	NULL	NULL	0	NULL	L1	NULL		bind	NULL				NP-1	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_21_23_6348_s_129	12456642	(d) G121S, a mutation that destroys homophilic binding, does not affect L1 binding to NP-1 or alter the ability of the chimera to induce the switch.	bind
13664	3	5075	7	10	NULL	0	NULL		NULL	mutant	does not affect	NULL		G121S		statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_23_6348_s_129	12456642	(d) G121S, a mutation that destroys homophilic binding, does not affect L1 binding to NP-1 or alter the ability of the chimera to induce the switch.	bind
13665	4	5075	7	NULL	NULL	0	NULL	chimera	NULL		induce	NULL				switch	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_21_23_6348_s_129	12456642	(d) G121S, a mutation that destroys homophilic binding, does not affect L1 binding to NP-1 or alter the ability of the chimera to induce the switch.	bind
13666	5	5075	7	10	NULL	0	NULL		NULL	mutant	does not alter	NULL		G121S		statement 4	NULL				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_23_6348_s_129	12456642	(d) G121S, a mutation that destroys homophilic binding, does not affect L1 binding to NP-1 or alter the ability of the chimera to induce the switch.	bind
13549	1	5076	6	NULL	NULL	NULL	NULL	GST-Prox1	GP	purified	bind					FGFR-3	GP	putative		Prox1 binding sequences of the promoter	NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_2_576_s_140	16291864	(D) Gel electrophoresis mobility shift assays  showed that the purified GST-Prox1 fusion protein (GST-ProxBD) but not the GST protein  alone binds to the putative Prox1 binding sequences found in the FGFR-3 promoter.	bind
13550	3	5076	6	NULL	NULL	NULL	NULL	GST-ProxBD	GP		is					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_2_576_s_140	16291864	(D) Gel electrophoresis mobility shift assays  showed that the purified GST-Prox1 fusion protein (GST-ProxBD) but not the GST protein  alone binds to the putative Prox1 binding sequences found in the FGFR-3 promoter.	bind
13595	4	5076	6	NULL	NULL	NULL	NULL	GST			does not bind		alone			FGFR-3	GP	putative		Prox1 binding sequences of the promoter	NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_2_576_s_140	16291864	(D) Gel electrophoresis mobility shift assays  showed that the purified GST-Prox1 fusion protein (GST-ProxBD) but not the GST protein  alone binds to the putative Prox1 binding sequences found in the FGFR-3 promoter.	bind
44672	2	5076	6	NULL	NULL	NULL	NULL	GST-Prox1	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_2_576_s_140	16291864	(D) Gel electrophoresis mobility shift assays  showed that the purified GST-Prox1 fusion protein (GST-ProxBD) but not the GST protein  alone binds to the putative Prox1 binding sequences found in the FGFR-3 promoter.	bind
13667	1	5076	7	10	NULL	0	NULL	GST-ProxBD	NULL	purified	bind	NULL				FGFR-3	NULL	putative		Prox1 binding sequences in the promoter of	NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_2_576_s_140	16291864	(D) Gel electrophoresis mobility shift assays  showed that the purified GST-Prox1 fusion protein (GST-ProxBD) but not the GST protein  alone binds to the putative Prox1 binding sequences found in the FGFR-3 promoter.	bind
13668	2	5076	7	10	NULL	0	NULL	GST	NULL		does not bind	NULL				FGFR-3	NULL	putative		Prox1 binding sequences in the promoter of	NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_2_576_s_140	16291864	(D) Gel electrophoresis mobility shift assays  showed that the purified GST-Prox1 fusion protein (GST-ProxBD) but not the GST protein  alone binds to the putative Prox1 binding sequences found in the FGFR-3 promoter.	bind
17774	4	5076	7	10	NULL	0	NULL	statement 3	NULL		is	NULL				GST-ProxBD	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_2_576_s_140	16291864	(D) Gel electrophoresis mobility shift assays  showed that the purified GST-Prox1 fusion protein (GST-ProxBD) but not the GST protein  alone binds to the putative Prox1 binding sequences found in the FGFR-3 promoter.	bind
44673	3	5076	7	10	NULL	0	NULL	GST-Prox1	NULL		is a type of	NULL				fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_2_576_s_140	16291864	(D) Gel electrophoresis mobility shift assays  showed that the purified GST-Prox1 fusion protein (GST-ProxBD) but not the GST protein  alone binds to the putative Prox1 binding sequences found in the FGFR-3 promoter.	bind
13551	1	5077	6	NULL	NULL	NULL	NULL	TR-RXR heterodimer	GP		bind									TRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2718_s_119	10733574	(D) Gel mobility shift assay of GST-DRIP205 binding to a TR-RXR heterodimer bound to a TRE in the presence of 10 6 M T3 (+) or ethanol ( ), as described in for panel C.	bind
13552	2	5077	6	NULL	NULL	NULL	NULL	GST-DRIP205	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2718_s_119	10733574	(D) Gel mobility shift assay of GST-DRIP205 binding to a TR-RXR heterodimer bound to a TRE in the presence of 10 6 M T3 (+) or ethanol ( ), as described in for panel C.	bind
13553	3	5077	6	NULL	NULL	NULL	NULL	statement 2	Process		occurs in presence of					T3	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2718_s_119	10733574	(D) Gel mobility shift assay of GST-DRIP205 binding to a TR-RXR heterodimer bound to a TRE in the presence of 10 6 M T3 (+) or ethanol ( ), as described in for panel C.	bind
13554	4	5077	6	NULL	NULL	NULL	NULL	statement 2	Process		occurs in presence of					ethanol	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2718_s_119	10733574	(D) Gel mobility shift assay of GST-DRIP205 binding to a TR-RXR heterodimer bound to a TRE in the presence of 10 6 M T3 (+) or ethanol ( ), as described in for panel C.	bind
13555	5	5077	6	NULL	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2718_s_119	10733574	(D) Gel mobility shift assay of GST-DRIP205 binding to a TR-RXR heterodimer bound to a TRE in the presence of 10 6 M T3 (+) or ethanol ( ), as described in for panel C.	bind
13669	1	5077	7	NULL	NULL	0	NULL	TR-RXR heterodimer	NULL		bind	NULL					NULL			TRE 	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2718_s_119	10733574	(D) Gel mobility shift assay of GST-DRIP205 binding to a TR-RXR heterodimer bound to a TRE in the presence of 10 6 M T3 (+) or ethanol ( ), as described in for panel C.	bind
13670	2	5077	7	NULL	NULL	0	NULL	GST-DRIP205	NULL		bind	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2718_s_119	10733574	(D) Gel mobility shift assay of GST-DRIP205 binding to a TR-RXR heterodimer bound to a TRE in the presence of 10 6 M T3 (+) or ethanol ( ), as described in for panel C.	bind
17776	5	5077	7	NULL	NULL	0	NULL	statement 3	NULL		is an alternative to	NULL				statement 4	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2718_s_119	10733574	(D) Gel mobility shift assay of GST-DRIP205 binding to a TR-RXR heterodimer bound to a TRE in the presence of 10 6 M T3 (+) or ethanol ( ), as described in for panel C.	bind
19969	3	5077	7	NULL	NULL	0	NULL	statement 2	NULL		occurs in the presence of	NULL				T3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2718_s_119	10733574	(D) Gel mobility shift assay of GST-DRIP205 binding to a TR-RXR heterodimer bound to a TRE in the presence of 10 6 M T3 (+) or ethanol ( ), as described in for panel C.	bind
19970	4	5077	7	NULL	NULL	0	NULL	statement 2	NULL		occurs in the presence of	NULL				ethanol	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2718_s_119	10733574	(D) Gel mobility shift assay of GST-DRIP205 binding to a TR-RXR heterodimer bound to a TRE in the presence of 10 6 M T3 (+) or ethanol ( ), as described in for panel C.	bind
13556	1	5079	6	NULL	NULL	NULL	NULL	GST-Akt	GP		bind					Grb10	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_4_979_s_180	11809791	(D) GST-Akt binds to Grb10 and Grb10deltaPH.	bind
13557	2	5079	6	NULL	NULL	NULL	NULL	GST-Akt	GP		bind					Grb10	GP		deltaPH		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_4_979_s_180	11809791	(D) GST-Akt binds to Grb10 and Grb10deltaPH.	bind
13672	1	5079	7	NULL	NULL	0	NULL	GST-Akt	NULL		binds	NULL				Grb10	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_4_979_s_180	11809791	(D) GST-Akt binds to Grb10 and Grb10deltaPH.	bind
13673	2	5079	7	NULL	NULL	0	NULL	GST-Akt	NULL		binds	NULL				Grb10	NULL		deltaPH		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_4_979_s_180	11809791	(D) GST-Akt binds to Grb10 and Grb10deltaPH.	bind
13598	1	5080	6	NULL	NULL	NULL	NULL	GST-p40PX	GP		bind		specifically			PI(3)P	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_1_35_s_197	12535519	(D) GST-p40PX and GST-FYVE3 bind specifically to PI(3)P. Hybond-C membranes spotted with the indicated lipids (pmoles) were incubated with GST-p40PX (10  g/ml) or GST-FYVE3 (10  g/ml) and extensively washed, and bound protein was detected by immunoblotting with an HRP-conjugated anti-GST antibody.	bind
13599	2	5080	6	NULL	NULL	NULL	NULL	GST-FYVE3	GP		bind		specifically			PI(3)P	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_1_35_s_197	12535519	(D) GST-p40PX and GST-FYVE3 bind specifically to PI(3)P. Hybond-C membranes spotted with the indicated lipids (pmoles) were incubated with GST-p40PX (10  g/ml) or GST-FYVE3 (10  g/ml) and extensively washed, and bound protein was detected by immunoblotting with an HRP-conjugated anti-GST antibody.	bind
13674	1	5080	7	NULL	NULL	0	NULL	GST-p40PX	NULL		bind	NULL	specifically			PI(3)P	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_35_s_197	12535519	(D) GST-p40PX and GST-FYVE3 bind specifically to PI(3)P. Hybond-C membranes spotted with the indicated lipids (pmoles) were incubated with GST-p40PX (10  g/ml) or GST-FYVE3 (10  g/ml) and extensively washed, and bound protein was detected by immunoblotting with an HRP-conjugated anti-GST antibody.	bind
13675	2	5080	7	NULL	NULL	0	NULL	GST-FYVE3	NULL		bind	NULL	specifically			PI(3)P	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_35_s_197	12535519	(D) GST-p40PX and GST-FYVE3 bind specifically to PI(3)P. Hybond-C membranes spotted with the indicated lipids (pmoles) were incubated with GST-p40PX (10  g/ml) or GST-FYVE3 (10  g/ml) and extensively washed, and bound protein was detected by immunoblotting with an HRP-conjugated anti-GST antibody.	bind
13558	1	5081	6	NULL	NULL	NULL	NULL	HNF-6	GP		bind					g6pc	GP	endogenous		promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_16_6037_s_90	16880515	(D) HNF-6 binds endogenous  g6pc promoter.	bind
13676	1	5081	7	NULL	NULL	0	NULL	HNF-6	NULL		binds	NULL				g6pc	NULL	endogenous		promoter	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_16_6037_s_90	16880515	(D) HNF-6 binds endogenous  g6pc promoter.	bind
13559	1	5082	6	NULL	NULL	NULL	NULL	HP1	GP		bind					H3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_4_729_s_210	11336697	(D) HP1  and Pc1/M33 bind to H3 in a CD integrity-dependent manner.	bind
13560	2	5082	6	NULL	NULL	NULL	NULL	Pc1/M33	GP		bind					H3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_4_729_s_210	11336697	(D) HP1  and Pc1/M33 bind to H3 in a CD integrity-dependent manner.	bind
13561	3	5082	6	NULL	NULL	NULL	NULL	statement 1	Process		is dependent on					CD 		integrity of 			NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_4_729_s_210	11336697	(D) HP1  and Pc1/M33 bind to H3 in a CD integrity-dependent manner.	bind
13562	4	5082	6	NULL	NULL	NULL	NULL	statement 2	Process		is dependent on					CD		integrity of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_4_729_s_210	11336697	(D) HP1  and Pc1/M33 bind to H3 in a CD integrity-dependent manner.	bind
13677	1	5082	7	NULL	NULL	0	NULL	HP1	NULL		bind	NULL				H3	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_7_4_729_s_210	11336697	(D) HP1  and Pc1/M33 bind to H3 in a CD integrity-dependent manner.	bind
13678	2	5082	7	NULL	NULL	0	NULL	Pc1/M33	NULL		bind	NULL				H3	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_7_4_729_s_210	11336697	(D) HP1  and Pc1/M33 bind to H3 in a CD integrity-dependent manner.	bind
13679	3	5082	7	NULL	NULL	0	NULL	statement 1	NULL		depends on	NULL				 CD  	NULL	integrity of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_4_729_s_210	11336697	(D) HP1  and Pc1/M33 bind to H3 in a CD integrity-dependent manner.	bind
13680	4	5082	7	NULL	NULL	0	NULL	statement 2	NULL		depends on	NULL				CD 	NULL	integrity of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_4_729_s_210	11336697	(D) HP1  and Pc1/M33 bind to H3 in a CD integrity-dependent manner.	bind
13563	1	5083	6	NULL	NULL	NULL	NULL	hTid-1	GP		bind		high affinity			IkappaB proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_1_44_s_131	15601829	(D) hTid-1 binds to IkappaB proteins with high affinity.	bind
13681	1	5083	7	NULL	NULL	0	NULL	hTid-1	NULL		binds	NULL	high affinity			IkappaB proteins	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_1_44_s_131	15601829	(D) hTid-1 binds to IkappaB proteins with high affinity.	bind
13597	1	5085	6	NULL	NULL	NULL	NULL	p53	GP	mutant	does not bind			S46A		p53AIP1	GP			p53BDS	NULL		NULL	NULL	NULL	NULL	gw60_cell_102_6_849_s_276	11030628	(D) Impaired binding activity of the  mutant p53 (S46A) protein to p53BDS of p53AIP1 but not p21Waf1.	bind
13772	2	5085	6	NULL	NULL	NULL	NULL	p53	GP	mutant	bind			S46A		p21Waf1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_102_6_849_s_276	11030628	(D) Impaired binding activity of the  mutant p53 (S46A) protein to p53BDS of p53AIP1 but not p21Waf1.	bind
13682	1	5085	7	NULL	NULL	0	NULL	p53	NULL	mutant	does not bind	NULL		S46A		p53AIP1	NULL			p53BDS	NULL		NULL	NULL	NULL	NULL	gw60_cell_102_6_849_s_276	11030628	(D) Impaired binding activity of the  mutant p53 (S46A) protein to p53BDS of p53AIP1 but not p21Waf1.	bind
13683	2	5085	7	NULL	NULL	0	NULL	p53	NULL	mutant	bind	NULL		S46A		p21Waf1	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_102_6_849_s_276	11030628	(D) Impaired binding activity of the  mutant p53 (S46A) protein to p53BDS of p53AIP1 but not p21Waf1.	bind
13564	1	5086	6	NULL	NULL	NULL	NULL	NFATc3	GP	full length	enhances					myogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6600_s_218	10938134	(D) In contrast, cotransfection of a expression vector encoding full-length NFATc3 produced a noticeable enhancement of myogenesis (extent of differentiation).	bind
13684	1	5086	7	NULL	NULL	0	NULL	NFATc3	NULL	full-length	enhance	NULL				myogenesis	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_17_6600_s_218	10938134	(D) In contrast, cotransfection of a expression vector encoding full-length NFATc3 produced a noticeable enhancement of myogenesis (extent of differentiation).	bind
13565	1	5087	6	NULL	NULL	NULL	NULL	PNT-P2	GP		bind					MAE	GP				NULL		NULL	NULL	NULL	NULL	gw60_development_130_5_845_s_342	12538513	(D) In the absence of signaling, PNT-P2 can bind to MAE and is prevented from activating transcription, either as a consequence of its interaction with MAE or because it is out competed by YAN, or both.	bind
13600	2	5087	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs in absence of					signaling	Process				NULL		NULL	NULL	NULL	NULL	gw60_development_130_5_845_s_342	12538513	(D) In the absence of signaling, PNT-P2 can bind to MAE and is prevented from activating transcription, either as a consequence of its interaction with MAE or because it is out competed by YAN, or both.	bind
13601	3	5087	6	NULL	NULL	NULL	NULL	PNT-P2	GP		activates					transcription	Process				NULL		NULL	NULL	NULL	NULL	gw60_development_130_5_845_s_342	12538513	(D) In the absence of signaling, PNT-P2 can bind to MAE and is prevented from activating transcription, either as a consequence of its interaction with MAE or because it is out competed by YAN, or both.	bind
13602	4	5087	6	NULL	NULL	NULL	NULL	statement 1	Process		prevents					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_development_130_5_845_s_342	12538513	(D) In the absence of signaling, PNT-P2 can bind to MAE and is prevented from activating transcription, either as a consequence of its interaction with MAE or because it is out competed by YAN, or both.	bind
13603	5	5087	6	NULL	NULL	NULL	NULL	PNT-P2	GP		bind					Yan	GP				NULL		NULL	NULL	NULL	NULL	gw60_development_130_5_845_s_342	12538513	(D) In the absence of signaling, PNT-P2 can bind to MAE and is prevented from activating transcription, either as a consequence of its interaction with MAE or because it is out competed by YAN, or both.	bind
13604	6	5087	6	NULL	NULL	NULL	NULL	statement 5	Process		prevents					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_development_130_5_845_s_342	12538513	(D) In the absence of signaling, PNT-P2 can bind to MAE and is prevented from activating transcription, either as a consequence of its interaction with MAE or because it is out competed by YAN, or both.	bind
13605	7	5087	6	NULL	NULL	NULL	NULL	statement 4	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_development_130_5_845_s_342	12538513	(D) In the absence of signaling, PNT-P2 can bind to MAE and is prevented from activating transcription, either as a consequence of its interaction with MAE or because it is out competed by YAN, or both.	bind
17717	8	5087	6	NULL	NULL	NULL	NULL	statement 5	GP		competes					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_development_130_5_845_s_342	12538513	(D) In the absence of signaling, PNT-P2 can bind to MAE and is prevented from activating transcription, either as a consequence of its interaction with MAE or because it is out competed by YAN, or both.	bind
13685	1	5087	7	NULL	NULL	0	NULL	PNT-P2	NULL		bind	NULL				MAE	NULL				NULL		0	NULL	NULL	NULL	gw60_development_130_5_845_s_342	12538513	(D) In the absence of signaling, PNT-P2 can bind to MAE and is prevented from activating transcription, either as a consequence of its interaction with MAE or because it is out competed by YAN, or both.	bind
13686	2	5087	7	NULL	NULL	0	NULL	statement 1	NULL		occurs in the absence of	NULL				signaling	NULL				NULL		NULL	NULL	NULL	NULL	gw60_development_130_5_845_s_342	12538513	(D) In the absence of signaling, PNT-P2 can bind to MAE and is prevented from activating transcription, either as a consequence of its interaction with MAE or because it is out competed by YAN, or both.	bind
13687	4	5087	7	NULL	NULL	0	NULL	statement 1	NULL		prevents	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_development_130_5_845_s_342	12538513	(D) In the absence of signaling, PNT-P2 can bind to MAE and is prevented from activating transcription, either as a consequence of its interaction with MAE or because it is out competed by YAN, or both.	bind
13688	5	5087	7	NULL	NULL	0	NULL	PNT-P2	NULL		bind	NULL				YAN	NULL				NULL		NULL	NULL	NULL	NULL	gw60_development_130_5_845_s_342	12538513	(D) In the absence of signaling, PNT-P2 can bind to MAE and is prevented from activating transcription, either as a consequence of its interaction with MAE or because it is out competed by YAN, or both.	bind
13689	6	5087	7	NULL	NULL	0	NULL	statement 4	NULL		occurs	NULL				statement 1	NULL	because of			NULL		NULL	NULL	NULL	NULL	gw60_development_130_5_845_s_342	12538513	(D) In the absence of signaling, PNT-P2 can bind to MAE and is prevented from activating transcription, either as a consequence of its interaction with MAE or because it is out competed by YAN, or both.	bind
13690	7	5087	7	NULL	NULL	0	NULL	statement 4	NULL		occurs 	NULL				statement 5	NULL	because of			NULL		NULL	NULL	NULL	NULL	gw60_development_130_5_845_s_342	12538513	(D) In the absence of signaling, PNT-P2 can bind to MAE and is prevented from activating transcription, either as a consequence of its interaction with MAE or because it is out competed by YAN, or both.	bind
13691	8	5087	7	NULL	NULL	0	NULL	statement 6	NULL		is an alternative to	NULL				statement 7	NULL				NULL		NULL	NULL	NULL	NULL	gw60_development_130_5_845_s_342	12538513	(D) In the absence of signaling, PNT-P2 can bind to MAE and is prevented from activating transcription, either as a consequence of its interaction with MAE or because it is out competed by YAN, or both.	bind
17777	3	5087	7	NULL	NULL	0	NULL	PNT-P2 	NULL		activates	NULL				transcription 	NULL				NULL		0	NULL	NULL	NULL	gw60_development_130_5_845_s_342	12538513	(D) In the absence of signaling, PNT-P2 can bind to MAE and is prevented from activating transcription, either as a consequence of its interaction with MAE or because it is out competed by YAN, or both.	bind
17781	9	5087	7	NULL	NULL	0	NULL	statement 1	NULL		compete with	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_development_130_5_845_s_342	12538513	(D) In the absence of signaling, PNT-P2 can bind to MAE and is prevented from activating transcription, either as a consequence of its interaction with MAE or because it is out competed by YAN, or both.	bind
13566	1	5088	6	NULL	NULL	NULL	NULL	RNA polymerase	GP		bind		selectively			P3	GP			promoter	NULL	wild-type aroP fragment	NULL	NULL	NULL	NULL	gw60_jbacteriol_180_20_5466_s_91	9765583	(d) In the presence of TyrR and tyrosine, RNA polymerase binds selectively to the P3 promoter on a wild-type  aroP fragment (P1+ P3+) (same pattern as for panel b).	bind
13567	2	5088	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs in presence of					TyrR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_20_5466_s_91	9765583	(d) In the presence of TyrR and tyrosine, RNA polymerase binds selectively to the P3 promoter on a wild-type  aroP fragment (P1+ P3+) (same pattern as for panel b).	bind
13568	3	5088	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs in presence of					tyrosine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_20_5466_s_91	9765583	(d) In the presence of TyrR and tyrosine, RNA polymerase binds selectively to the P3 promoter on a wild-type  aroP fragment (P1+ P3+) (same pattern as for panel b).	bind
13692	1	5088	7	NULL	NULL	0	NULL	RNA polymerase	NULL		binds	NULL	selectively			P3	NULL			promoter	NULL	wild-type aroP fragment 	0	NULL	NULL	NULL	gw60_jbacteriol_180_20_5466_s_91	9765583	(d) In the presence of TyrR and tyrosine, RNA polymerase binds selectively to the P3 promoter on a wild-type  aroP fragment (P1+ P3+) (same pattern as for panel b).	bind
13693	2	5088	7	NULL	NULL	0	NULL	statement 1	NULL		occurs in the presence of	NULL				TyrR	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_20_5466_s_91	9765583	(d) In the presence of TyrR and tyrosine, RNA polymerase binds selectively to the P3 promoter on a wild-type  aroP fragment (P1+ P3+) (same pattern as for panel b).	bind
13694	3	5088	7	NULL	NULL	0	NULL	statement 1	NULL		occurs in the presence of	NULL				tyrosine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_20_5466_s_91	9765583	(d) In the presence of TyrR and tyrosine, RNA polymerase binds selectively to the P3 promoter on a wild-type  aroP fragment (P1+ P3+) (same pattern as for panel b).	bind
13569	1	5089	6	NULL	NULL	NULL	NULL	mto1p	GP	truncated	bind					GST-mto2p	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molbiolcell_16_6_3040_s_186	15659644	(D) In vitro binding  of mto1p truncations to GST-mto2p by pull-down assays.	bind
13695	1	5089	7	NULL	NULL	0	NULL	mto1p	NULL	truncated	binds	NULL				GST-mto2p	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw70_molbiolcell_16_6_3040_s_186	15659644	(D) In vitro binding  of mto1p truncations to GST-mto2p by pull-down assays.	bind
13570	2	5090	6	NULL	NULL	NULL	NULL	Pex19p	GP		bind					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molbiolcell_15_7_3406_s_111	15133130	(D) In vitro binding of Pex19p to Pex13p-derived synthetic peptides.	bind
44674	1	5090	6	NULL	NULL	NULL	NULL	synthetic peptides			is derived from					Pex13p	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_7_3406_s_111	15133130	(D) In vitro binding of Pex19p to Pex13p-derived synthetic peptides.	bind
13696	2	5090	7	10	NULL	0	NULL	Pex19p	NULL		bind	NULL				statement 1	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molbiolcell_15_7_3406_s_111	15133130	(D) In vitro binding of Pex19p to Pex13p-derived synthetic peptides.	bind
44675	1	5090	7	10	NULL	0	NULL	synthetic peptides	NULL		is derived from	NULL				Pex13p	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_7_3406_s_111	15133130	(D) In vitro binding of Pex19p to Pex13p-derived synthetic peptides.	bind
13571	1	5091	6	NULL	NULL	NULL	NULL	KIF13A	GP	purified;;recombinant	bind					beta1-adaptin	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_cell_103_4_569_s_133	11106728	(D) In vitro binding of purified recombinant KIF13A and beta1-adaptin.	bind
13697	1	5091	7	10	NULL	0	NULL	KIF13A	NULL	purified;;recombinant	bind	NULL				beta1-adaptin	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_cell_103_4_569_s_133	11106728	(D) In vitro binding of purified recombinant KIF13A and beta1-adaptin.	bind
13572	1	5092	6	NULL	NULL	NULL	NULL	v-Rel proteins	GP	mutant	bind					DNA	NucleicAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_23_5_1520_s_212	12588973	(D) In vitro DNA-binding activity of mutant v-Rel proteins.	bind
13698	1	5092	7	NULL	NULL	0	NULL	v-Rel protein	NULL	mutant	bind	NULL				DNA	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_molcellbiol_23_5_1520_s_212	12588973	(D) In vitro DNA-binding activity of mutant v-Rel proteins.	bind
13573	1	5093	6	NULL	NULL	NULL	NULL	cyclin D1	GP		bind					GAL-ER	CellComponent				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_cell_88_3_405_s_212	9039267	(D) In vivo binding between cyclin D1 and  GAL-ER fusion proteins.	bind
44676	2	5093	6	NULL	NULL	NULL	NULL	GAL-ER	CellComponent		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_88_3_405_s_212	9039267	(D) In vivo binding between cyclin D1 and  GAL-ER fusion proteins.	bind
13699	1	5093	7	10	NULL	0	NULL	cyclin D1	NULL		bind	NULL				GAL-ER	NULL				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_cell_88_3_405_s_212	9039267	(D) In vivo binding between cyclin D1 and  GAL-ER fusion proteins.	bind
44677	2	5093	7	10	NULL	0	NULL	GAL-ER	NULL		is a type of	NULL				fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_88_3_405_s_212	9039267	(D) In vivo binding between cyclin D1 and  GAL-ER fusion proteins.	bind
13574	1	5094	6	NULL	NULL	NULL	NULL	Ey	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_3_297_s_181	10198632	(D) Increased DNA-binding activity of Ey due to a single amino acid substitution.	bind
13575	2	5094	6	NULL	NULL	NULL	NULL	Ey	GP	single amino acid substitution of	increases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_3_297_s_181	10198632	(D) Increased DNA-binding activity of Ey due to a single amino acid substitution.	bind
13700	1	5094	7	NULL	NULL	0	NULL	Ey 	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_3_3_297_s_181	10198632	(D) Increased DNA-binding activity of Ey due to a single amino acid substitution.	bind
13701	2	5094	7	10	NULL	0	NULL	Ey	NULL	single amino acid substitution of	increases	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_3_297_s_181	10198632	(D) Increased DNA-binding activity of Ey due to a single amino acid substitution.	bind
13576	1	5095	6	NULL	NULL	NULL	NULL	p53	GP		bind					Cyclin A1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_8917_s_195	15456866	(D) Increased p53 binding to the cyclin  A1 promoter following irradiation.	bind
13577	2	5095	6	NULL	NULL	NULL	NULL	statement 1	Process		increases following					irradiation					NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_8917_s_195	15456866	(D) Increased p53 binding to the cyclin  A1 promoter following irradiation.	bind
13702	1	5095	7	NULL	NULL	0	NULL	p53	NULL		bind	NULL				cyclin A1	NULL			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_8917_s_195	15456866	(D) Increased p53 binding to the cyclin  A1 promoter following irradiation.	bind
13703	2	5095	7	NULL	NULL	0	NULL	statement 1	NULL		is increased upon	NULL				irradiation	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_20_8917_s_195	15456866	(D) Increased p53 binding to the cyclin  A1 promoter following irradiation.	bind
13578	1	5096	6	NULL	NULL	NULL	NULL	mSin3a	GP	endogenous	bind					Elk-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_8_2802_s_281	11283259	(D) Inducible binding of endogenous mSin3A to Elk-1 following EGF induction.	bind
13579	2	5096	6	NULL	NULL	NULL	NULL	EGF	GP		induces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_8_2802_s_281	11283259	(D) Inducible binding of endogenous mSin3A to Elk-1 following EGF induction.	bind
13704	1	5096	7	NULL	NULL	0	NULL	mSin3A	NULL	endogenous	bind	NULL				 Elk-1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_8_2802_s_281	11283259	(D) Inducible binding of endogenous mSin3A to Elk-1 following EGF induction.	bind
13705	2	5096	7	NULL	NULL	0	NULL	EGF	NULL		induce	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_8_2802_s_281	11283259	(D) Inducible binding of endogenous mSin3A to Elk-1 following EGF induction.	bind
13580	1	5097	6	NULL	NULL	NULL	NULL	Hsp70	GP		bind					macrophages	Cell	human			NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_3_353_s_45	12354387	(D) Inhibition of Hsp70 binding to human macrophages (M ) and peripheral blood myeloid DC.	bind
13581	2	5097	6	NULL	NULL	NULL	NULL	Hsp70	GP		bind					peripheral blood myeloid DC	Cell				NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_3_353_s_45	12354387	(D) Inhibition of Hsp70 binding to human macrophages (M ) and peripheral blood myeloid DC.	bind
17718	3	5097	6	NULL	NULL	0	NULL	M	NULL		is	NULL				macrophages	NULL				NULL		0	NULL	NULL	NULL	gw60_immunity_17_3_353_s_45	12354387	(D) Inhibition of Hsp70 binding to human macrophages (M ) and peripheral blood myeloid DC.	bind
13706	1	5097	7	NULL	NULL	0	NULL	Hsp70	NULL		bind	NULL				macrophages	NULL	human			NULL		0	NULL	NULL	NULL	gw60_immunity_17_3_353_s_45	12354387	(D) Inhibition of Hsp70 binding to human macrophages (M ) and peripheral blood myeloid DC.	bind
13707	2	5097	7	NULL	NULL	0	NULL	Hsp70	NULL		bind	NULL				peripheral blood myeloid DC	NULL				NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_3_353_s_45	12354387	(D) Inhibition of Hsp70 binding to human macrophages (M ) and peripheral blood myeloid DC.	bind
13708	3	5097	7	NULL	NULL	0	NULL	macrophages	NULL		is	NULL				M	NULL				NULL		0	NULL	NULL	NULL	gw60_immunity_17_3_353_s_45	12354387	(D) Inhibition of Hsp70 binding to human macrophages (M ) and peripheral blood myeloid DC.	bind
13582	1	5098	6	NULL	NULL	NULL	NULL	MyoD	GP		bind					Tncs	GP			regulatory region	NULL		NULL	NULL	NULL	NULL	gw60_molcell_9_3_587_s_199	11931766	(D) Inhibition of p38 kinase does not alter MyoD binding to the  Tncs regulatory region as assessed by ChIP analysis of SB 203580-treated samples.	bind
13583	2	5098	6	NULL	NULL	NULL	NULL	p38 kinase	GP	inhibition of	does not alter					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_9_3_587_s_199	11931766	(D) Inhibition of p38 kinase does not alter MyoD binding to the  Tncs regulatory region as assessed by ChIP analysis of SB 203580-treated samples.	bind
13709	1	5098	7	NULL	NULL	0	NULL	MyoD	NULL		bind	NULL				Tncs	NULL			regulatory region	NULL		0	NULL	NULL	NULL	gw60_molcell_9_3_587_s_199	11931766	(D) Inhibition of p38 kinase does not alter MyoD binding to the  Tncs regulatory region as assessed by ChIP analysis of SB 203580-treated samples.	bind
13710	2	5098	7	NULL	NULL	0	NULL	p38 kinase	NULL	inhibition of	does not alter	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_9_3_587_s_199	11931766	(D) Inhibition of p38 kinase does not alter MyoD binding to the  Tncs regulatory region as assessed by ChIP analysis of SB 203580-treated samples.	bind
13606	1	5099	6	NULL	NULL	NULL	NULL	Tob	GP		interacts with					Smad1	GP	deletion mutants			NULL		NULL	NULL	NULL	NULL	gw60_cell_103_7_1085_s_192	11163184	(D) Interaction of  Tob with various Smad1 deletion mutants.	bind
13711	1	5099	7	NULL	NULL	0	NULL	Tob	NULL		interacts with	NULL				Smad1	NULL	deletion mutant			NULL		NULL	NULL	NULL	NULL	gw60_cell_103_7_1085_s_192	11163184	(D) Interaction of  Tob with various Smad1 deletion mutants.	bind
13607	1	5100	6	NULL	NULL	NULL	NULL	L-periaxin	GP		bind			binding domain		DRP2	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_neuron_30_3_677_s_45	11430802	(D) Interaction of the binding domains of L-periaxin and DRP2 in vitro.	bind
13712	1	5100	7	NULL	NULL	0	NULL	L-periaxin	NULL		bind	NULL		binding domain		DRP2	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_neuron_30_3_677_s_45	11430802	(D) Interaction of the binding domains of L-periaxin and DRP2 in vitro.	bind
13608	1	5102	6	NULL	NULL	NULL	NULL	Kap121p	GP		bind					Nup53p	GP				NULL	NPC	NULL	NULL	NULL	NULL	gw60_cellbiol_159_2_267_s_237	12403813	(D) Kap121p bound to Nup53p at the NPC could then be released by stochastic changes that allow Nup53p to bind Nup170p.	bind
13609	2	5102	6	NULL	NULL	NULL	NULL	Nup53p	GP		released by					stochastic changes	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_2_267_s_237	12403813	(D) Kap121p bound to Nup53p at the NPC could then be released by stochastic changes that allow Nup53p to bind Nup170p.	bind
13610	3	5102	6	NULL	NULL	NULL	NULL	Nup53p	GP		bind					Nup170p	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_2_267_s_237	12403813	(D) Kap121p bound to Nup53p at the NPC could then be released by stochastic changes that allow Nup53p to bind Nup170p.	bind
13611	4	5102	6	NULL	NULL	NULL	NULL	statement 2	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_2_267_s_237	12403813	(D) Kap121p bound to Nup53p at the NPC could then be released by stochastic changes that allow Nup53p to bind Nup170p.	bind
13713	1	5102	7	NULL	NULL	0	NULL	Kap121p 	NULL		bind	NULL				Nup53p	NULL				NULL	at NPC	NULL	NULL	NULL	NULL	gw60_cellbiol_159_2_267_s_237	12403813	(D) Kap121p bound to Nup53p at the NPC could then be released by stochastic changes that allow Nup53p to bind Nup170p.	bind
13714	2	5102	7	NULL	NULL	0	NULL	Nup53p	NULL		bind	NULL				Nup170p	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_159_2_267_s_237	12403813	(D) Kap121p bound to Nup53p at the NPC could then be released by stochastic changes that allow Nup53p to bind Nup170p.	bind
13715	3	5102	7	NULL	NULL	0	NULL	Nup53p	NULL	release of	occurs by	NULL				stochastic changes	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_2_267_s_237	12403813	(D) Kap121p bound to Nup53p at the NPC could then be released by stochastic changes that allow Nup53p to bind Nup170p.	bind
44722	4	5102	7	NULL	NULL	0	NULL	statement 3	NULL		leads to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_159_2_267_s_237	12403813	(D) Kap121p bound to Nup53p at the NPC could then be released by stochastic changes that allow Nup53p to bind Nup170p.	bind
13612	1	5103	6	NULL	NULL	NULL	NULL	Grb2	GP		bind			SH3 domain		Sos-1	GP		proline-rich COOH-terminal (aa 1131 - 1333)		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_156_1_125_s_86	11777939	(D) Kinetic analysis and rate constants for the binding of the SH3 domains of Grb2 and E3b1 to the proline-rich COOH-terminal of Sos-1 (aa 1131 - 1333).	bind
13613	2	5103	6	NULL	NULL	NULL	NULL	E3b1	GP		bind			SH3 domain		Sos-1	GP		proline-rich COOH-terminal (aa 1131 - 1333)		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_156_1_125_s_86	11777939	(D) Kinetic analysis and rate constants for the binding of the SH3 domains of Grb2 and E3b1 to the proline-rich COOH-terminal of Sos-1 (aa 1131 - 1333).	bind
13716	1	5103	7	10	NULL	0	NULL	Grb2	NULL		bind	NULL		SH3 domain		Sos-1	NULL		proline-rich COOH-terminal (aa 1131 - 1333)		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_156_1_125_s_86	11777939	(D) Kinetic analysis and rate constants for the binding of the SH3 domains of Grb2 and E3b1 to the proline-rich COOH-terminal of Sos-1 (aa 1131 - 1333).	bind
13717	2	5103	7	10	NULL	0	NULL	E3b1	NULL		bind	NULL		SH3 domain		Sos-1	NULL		proline-rich COOH-terminal (aa 1131 - 1333)		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_156_1_125_s_86	11777939	(D) Kinetic analysis and rate constants for the binding of the SH3 domains of Grb2 and E3b1 to the proline-rich COOH-terminal of Sos-1 (aa 1131 - 1333).	bind
13621	1	5104	6	NULL	NULL	NULL	NULL	KLF7	GP		bind					p27Kip1	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5699_s_253	15964824	(d) KLF7 binds in vivo to the  p27 kip1 promoter.	bind
13718	1	5104	7	NULL	NULL	0	NULL	KLF7	NULL		bind	NULL				p27 kip1	NULL			promoter	NULL	in vivo	0	NULL	NULL	NULL	gw70_molcellbiol_25_13_5699_s_253	15964824	(d) KLF7 binds in vivo to the  p27 kip1 promoter.	bind
13623	1	5108	6	NULL	NULL	NULL	NULL	Pdcd4	GP		bind					eIF4A	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_1_26_s_163	12482958	(D) Mammalian two-hybrid assay of Pdcd4 binding to eIF4A.	bind
13719	1	5108	7	NULL	NULL	0	NULL	Pdcd4	NULL		bind	NULL				eIF4A	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_1_26_s_163	12482958	(D) Mammalian two-hybrid assay of Pdcd4 binding to eIF4A.	bind
13624	1	5110	6	NULL	NULL	NULL	NULL	MBP-3	GP		does not bind					dsRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_6_1908_s_268	11238927	(D) MBP-3 cannot bind dsRNA. MBP, MBP-3, and wt PACT were tested for poly(I-C)-agarose binding activity.	bind
13721	1	5110	7	NULL	NULL	0	NULL	MBP-3	NULL		does not bind	NULL				dsRNA	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_6_1908_s_268	11238927	(D) MBP-3 cannot bind dsRNA. MBP, MBP-3, and wt PACT were tested for poly(I-C)-agarose binding activity.	bind
13626	1	5111	6	NULL	NULL	NULL	NULL	MBP-3	GP		does not bind					DD	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_6_1908_s_332	11238927	(D) MBP-3 cannot bind to DD.	bind
13722	1	5111	7	NULL	NULL	0	NULL	MBP-3	NULL		does not bind	NULL				DD	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_6_1908_s_332	11238927	(D) MBP-3 cannot bind to DD.	bind
13627	1	5112	6	NULL	NULL	NULL	NULL	MKK3	GP		stimulates					NFATc-CBP	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6442_s_305	12944472	(D) MKK3(E) stimulated NFATc-CBP binding.	bind
13724	1	5112	7	NULL	NULL	0	NULL	MKK3	NULL		stimulate	NULL				NFATc-CBP	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6442_s_305	12944472	(D) MKK3(E) stimulated NFATc-CBP binding.	bind
13628	1	5113	6	NULL	NULL	NULL	NULL	IP3	GP		bind					PRR-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_9_7_829_s_149	12144927	(D) Molecular models of IP3 and IP6 bound to PRR-2.	bind
13629	2	5113	6	NULL	NULL	NULL	NULL	IP6	GP		bind					PRR-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_9_7_829_s_149	12144927	(D) Molecular models of IP3 and IP6 bound to PRR-2.	bind
13725	1	5113	7	NULL	NULL	0	NULL	IP3	NULL		bind	NULL				PRR-2	NULL				NULL		0	NULL	NULL	NULL	gw60_chembiol_9_7_829_s_149	12144927	(D) Molecular models of IP3 and IP6 bound to PRR-2.	bind
13726	2	5113	7	NULL	NULL	0	NULL	IP6	NULL		bind	NULL				PRR-2	NULL				NULL		0	NULL	NULL	NULL	gw60_chembiol_9_7_829_s_149	12144927	(D) Molecular models of IP3 and IP6 bound to PRR-2.	bind
13631	1	5114	6	NULL	NULL	NULL	NULL	APP	GP		bind					KLC	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_28_2_449_s_137	11144355	(D) Monoclonal antibody to the TPR domain of KLC (KLC-All) inhibits APP binding to KLC.	bind
13632	2	5114	6	NULL	NULL	NULL	NULL	KLC-All	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_28_2_449_s_137	11144355	(D) Monoclonal antibody to the TPR domain of KLC (KLC-All) inhibits APP binding to KLC.	bind
13633	3	5114	6	NULL	NULL	NULL	NULL	KLC-All	GP		is					monoclonal antibody to the TPR domain of KLC	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_28_2_449_s_137	11144355	(D) Monoclonal antibody to the TPR domain of KLC (KLC-All) inhibits APP binding to KLC.	bind
13727	1	5114	7	NULL	NULL	0	NULL	APP	NULL		bind	NULL				KLC	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_28_2_449_s_137	11144355	(D) Monoclonal antibody to the TPR domain of KLC (KLC-All) inhibits APP binding to KLC.	bind
13728	2	5114	7	10	NULL	0	NULL	KLC-All	NULL		inhibits	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuron_28_2_449_s_137	11144355	(D) Monoclonal antibody to the TPR domain of KLC (KLC-All) inhibits APP binding to KLC.	bind
17782	3	5114	7	10	NULL	0	NULL	KLC-All	NULL		is	NULL				monoclonal antibody to the TPR domain of KLC	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuron_28_2_449_s_137	11144355	(D) Monoclonal antibody to the TPR domain of KLC (KLC-All) inhibits APP binding to KLC.	bind
14085	1	5115	6	NULL	NULL	NULL	NULL	IFN-gamma	GP		induce					Stat1alpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_71_3_1442_s_205	12595462	(D) Moreover, neither IFN-gamma-induced Stat1alpha nor IFN-gamma-induced IRF-1 bound either NF-kappaB-binding site, although, as expected, there was binding to GAS and ISRE sites, respectively.	bind
14086	2	5115	6	NULL	NULL	NULL	NULL	IFN-gamma	GP		induce					IRF-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_71_3_1442_s_205	12595462	(D) Moreover, neither IFN-gamma-induced Stat1alpha nor IFN-gamma-induced IRF-1 bound either NF-kappaB-binding site, although, as expected, there was binding to GAS and ISRE sites, respectively.	bind
14087	3	5115	6	NULL	NULL	NULL	NULL	statement 1	Process		does not bind									NF-kappaB-binding site	NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_71_3_1442_s_205	12595462	(D) Moreover, neither IFN-gamma-induced Stat1alpha nor IFN-gamma-induced IRF-1 bound either NF-kappaB-binding site, although, as expected, there was binding to GAS and ISRE sites, respectively.	bind
14088	4	5115	6	NULL	NULL	NULL	NULL	statement 2	Process		does not bind									NF-kappaB-binding site	NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_71_3_1442_s_205	12595462	(D) Moreover, neither IFN-gamma-induced Stat1alpha nor IFN-gamma-induced IRF-1 bound either NF-kappaB-binding site, although, as expected, there was binding to GAS and ISRE sites, respectively.	bind
14089	5	5115	6	NULL	NULL	NULL	NULL	statement 1	Process		bind									GAS site	NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_71_3_1442_s_205	12595462	(D) Moreover, neither IFN-gamma-induced Stat1alpha nor IFN-gamma-induced IRF-1 bound either NF-kappaB-binding site, although, as expected, there was binding to GAS and ISRE sites, respectively.	bind
14090	6	5115	6	NULL	NULL	NULL	NULL	statement 2	Process		bind									ISRE site	NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_71_3_1442_s_205	12595462	(D) Moreover, neither IFN-gamma-induced Stat1alpha nor IFN-gamma-induced IRF-1 bound either NF-kappaB-binding site, although, as expected, there was binding to GAS and ISRE sites, respectively.	bind
13729	1	5115	7	NULL	NULL	0	NULL	IFN-gamma	NULL		induce	NULL				Stat1alpha 	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_71_3_1442_s_205	12595462	(D) Moreover, neither IFN-gamma-induced Stat1alpha nor IFN-gamma-induced IRF-1 bound either NF-kappaB-binding site, although, as expected, there was binding to GAS and ISRE sites, respectively.	bind
13730	2	5115	7	NULL	NULL	0	NULL	IFN-gamma	NULL		induce	NULL				IRF-1	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_71_3_1442_s_205	12595462	(D) Moreover, neither IFN-gamma-induced Stat1alpha nor IFN-gamma-induced IRF-1 bound either NF-kappaB-binding site, although, as expected, there was binding to GAS and ISRE sites, respectively.	bind
13731	3	5115	7	NULL	NULL	0	NULL	statement 1	NULL		does not bind	NULL					NULL			NF-kappaB binding site	NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_71_3_1442_s_205	12595462	(D) Moreover, neither IFN-gamma-induced Stat1alpha nor IFN-gamma-induced IRF-1 bound either NF-kappaB-binding site, although, as expected, there was binding to GAS and ISRE sites, respectively.	bind
13732	4	5115	7	NULL	NULL	0	NULL	statement 2	NULL		does not bind	NULL					NULL			NF-kappaB binding site	NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_71_3_1442_s_205	12595462	(D) Moreover, neither IFN-gamma-induced Stat1alpha nor IFN-gamma-induced IRF-1 bound either NF-kappaB-binding site, although, as expected, there was binding to GAS and ISRE sites, respectively.	bind
13733	5	5115	7	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL					NULL			GAS site	NULL		0	NULL	NULL	NULL	gw60_infectimmun_71_3_1442_s_205	12595462	(D) Moreover, neither IFN-gamma-induced Stat1alpha nor IFN-gamma-induced IRF-1 bound either NF-kappaB-binding site, although, as expected, there was binding to GAS and ISRE sites, respectively.	bind
13734	6	5115	7	10	NULL	0	NULL	statement 2	NULL		bind	NULL					NULL			ISRE site	NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_71_3_1442_s_205	12595462	(D) Moreover, neither IFN-gamma-induced Stat1alpha nor IFN-gamma-induced IRF-1 bound either NF-kappaB-binding site, although, as expected, there was binding to GAS and ISRE sites, respectively.	bind
13635	1	5117	6	NULL	NULL	NULL	NULL	transcription factor	GP		bind									AP/dE composite element	NULL	nuclear extracts from hormone-treated hBC cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_16_7260_s_185	15282324	(D) Mutant analysis of in vitro  transcription factor binding to the AP/dE composite element by EMSAs with nuclear  extracts from hormone-treated hBC cells.	bind
13737	1	5117	7	10	NULL	0	NULL	transcription factor	NULL		bind	NULL					NULL			AP/dE composite element 	NULL	nuclear extracts from hormone-treated hBC cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_16_7260_s_185	15282324	(D) Mutant analysis of in vitro  transcription factor binding to the AP/dE composite element by EMSAs with nuclear  extracts from hormone-treated hBC cells.	bind
13636	1	5118	6	NULL	NULL	NULL	NULL	Brf1	GP		bind					C-DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_231	16880507	(D) Mutant peptides do not inhibit Brf1 binding to C-DNA.	bind
13638	2	5118	6	NULL	NULL	NULL	NULL	peptides	GP	mutant	do not inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_231	16880507	(D) Mutant peptides do not inhibit Brf1 binding to C-DNA.	bind
13738	1	5118	7	NULL	NULL	0	NULL	Brf1	NULL		bind	NULL				C-DNA	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_231	16880507	(D) Mutant peptides do not inhibit Brf1 binding to C-DNA.	bind
13739	2	5118	7	NULL	NULL	0	NULL	peptides	NULL	mutant	does not inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_231	16880507	(D) Mutant peptides do not inhibit Brf1 binding to C-DNA.	bind
13640	1	5119	6	NULL	NULL	NULL	NULL	Nck	GP		bind								PRS		NULL		NULL	NULL	NULL	NULL	gw60_cell_109_7_901_s_86	12110186	(D) Nck binds to the PRS.	bind
13740	1	5119	7	NULL	NULL	0	NULL	Nck	NULL		binds	NULL					NULL		PRS		NULL		NULL	NULL	NULL	NULL	gw60_cell_109_7_901_s_86	12110186	(D) Nck binds to the PRS.	bind
13641	1	5120	6	NULL	NULL	NULL	NULL	NFAT5	GP		bind					aldose reductase	GP			enhancer	NULL	living cells	NULL	NULL	NULL	NULL	gw60_immunity_15_1_47_s_167	11485737	(D) NFAT5 binds to the aldose reductase enhancer and the  TNF  proximal promoter in living cells.	bind
13642	2	5120	6	NULL	NULL	NULL	NULL	NFAT5	GP		bind					TNF	GP			proximal promoter	NULL	living cells	NULL	NULL	NULL	NULL	gw60_immunity_15_1_47_s_167	11485737	(D) NFAT5 binds to the aldose reductase enhancer and the  TNF  proximal promoter in living cells.	bind
13741	1	5120	7	NULL	NULL	0	NULL	NFAT5	NULL		bind	NULL				aldose reductase	NULL			enhancer	NULL	living cells	0	NULL	NULL	NULL	gw60_immunity_15_1_47_s_167	11485737	(D) NFAT5 binds to the aldose reductase enhancer and the  TNF  proximal promoter in living cells.	bind
13742	2	5120	7	NULL	NULL	0	NULL	NFAT5	NULL		bind	NULL				TNF	NULL			proximal promoter	NULL	living cells	0	NULL	NULL	NULL	gw60_immunity_15_1_47_s_167	11485737	(D) NFAT5 binds to the aldose reductase enhancer and the  TNF  proximal promoter in living cells.	bind
13643	1	5121	6	NULL	NULL	NULL	NULL	NORE1	GP		bind					MST1	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_4_253_s_67	11864565	(D) NORE1 binds MST 1, but not related kinases.	bind
13644	2	5121	6	NULL	NULL	NULL	NULL	NORE1	GP		does not bind					MST1 related kinases	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_4_253_s_67	11864565	(D) NORE1 binds MST 1, but not related kinases.	bind
13743	1	5121	7	NULL	NULL	0	NULL	NORE1	NULL		binds	NULL				MST 1	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_12_4_253_s_67	11864565	(D) NORE1 binds MST 1, but not related kinases.	bind
13744	2	5121	7	NULL	NULL	0	NULL	NORE1	NULL		does not bind	NULL				MST 1 related kinases	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_12_4_253_s_67	11864565	(D) NORE1 binds MST 1, but not related kinases.	bind
13645	1	5123	6	NULL	NULL	0	NULL	Npap60	NULL		bind	NULL				importin-alpha isoforms	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_110_3_349_s_141	12176322	(D) Npap60 binds several importin-alpha isoforms.	bind
13745	1	5123	7	NULL	NULL	0	NULL	Npap60	NULL		binds	NULL				importin-alpha isoform	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_110_3_349_s_141	12176322	(D) Npap60 binds several importin-alpha isoforms.	bind
14091	1	5125	6	NULL	NULL	NULL	NULL	NFAT	GP		bind					PPARgamma2 gene	GP			proximal NFAT binding element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3892_s_361	11997522	(D) Nuclear extracts prepared from differentiated 3T3-L1 adipocytes form NFAT-DNA complexes on the proximal and the distal NFAT binding elements of the PPARgamma2 gene.	bind
14092	2	5125	6	NULL	NULL	NULL	NULL	NFAT	GP		bind					PPARgamma2 gene	GP			distal NFAT binding element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3892_s_361	11997522	(D) Nuclear extracts prepared from differentiated 3T3-L1 adipocytes form NFAT-DNA complexes on the proximal and the distal NFAT binding elements of the PPARgamma2 gene.	bind
53081	3	5125	6	NULL	NULL	NULL	NULL	nuclear extracts	CellComponent		are prepared from					3T3-L1 adipocytes	Cell	differentiated			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3892_s_361	11997522	(D) Nuclear extracts prepared from differentiated 3T3-L1 adipocytes form NFAT-DNA complexes on the proximal and the distal NFAT binding elements of the PPARgamma2 gene.	bind
53082	4	5125	6	NULL	NULL	NULL	NULL	statement 3	Process		form					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3892_s_361	11997522	(D) Nuclear extracts prepared from differentiated 3T3-L1 adipocytes form NFAT-DNA complexes on the proximal and the distal NFAT binding elements of the PPARgamma2 gene.	bind
53083	5	5125	6	NULL	NULL	NULL	NULL	statement 3	Process		form					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3892_s_361	11997522	(D) Nuclear extracts prepared from differentiated 3T3-L1 adipocytes form NFAT-DNA complexes on the proximal and the distal NFAT binding elements of the PPARgamma2 gene.	bind
13746	1	5125	7	10	NULL	0	NULL	NFAT	NULL		bind	NULL				PPARgamma2	NULL			proximal NFAT binding elements	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3892_s_361	11997522	(D) Nuclear extracts prepared from differentiated 3T3-L1 adipocytes form NFAT-DNA complexes on the proximal and the distal NFAT binding elements of the PPARgamma2 gene.	bind
17784	2	5125	7	10	NULL	0	NULL	NFAT	NULL		bind	NULL				PPARgamma2	NULL			distal NFAT binding element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3892_s_361	11997522	(D) Nuclear extracts prepared from differentiated 3T3-L1 adipocytes form NFAT-DNA complexes on the proximal and the distal NFAT binding elements of the PPARgamma2 gene.	bind
53084	3	5125	7	10	NULL	0	NULL	nuclear extracts	NULL		are prepared from	NULL				3T3-L1 adipocytes	NULL	differentiated			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_11_3892_s_361	11997522	(D) Nuclear extracts prepared from differentiated 3T3-L1 adipocytes form NFAT-DNA complexes on the proximal and the distal NFAT binding elements of the PPARgamma2 gene.	bind
53085	4	5125	7	10	NULL	0	NULL	statement 3	NULL		form	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_11_3892_s_361	11997522	(D) Nuclear extracts prepared from differentiated 3T3-L1 adipocytes form NFAT-DNA complexes on the proximal and the distal NFAT binding elements of the PPARgamma2 gene.	bind
53086	5	5125	7	10	NULL	0	NULL	statement 3	NULL		form	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_11_3892_s_361	11997522	(D) Nuclear extracts prepared from differentiated 3T3-L1 adipocytes form NFAT-DNA complexes on the proximal and the distal NFAT binding elements of the PPARgamma2 gene.	bind
13646	1	5126	6	NULL	NULL	NULL	NULL	Nup60p	GP		bind					Prp20p	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_937_s_193	11535617	(D) Nup60p binds Prp20p.	bind
13790	1	5126	7	NULL	NULL	0	NULL	Nup60p	NULL		binds	NULL				Prp20p	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_154_5_937_s_193	11535617	(D) Nup60p binds Prp20p.	bind
13650	1	5128	6	NULL	NULL	NULL	NULL	Bcl2	GP	hypophosphorylated	bind		only			Bax	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_6_3509_s_128	9584191	(D) Only hypophosphorylated Bcl2 binds to Bax.	bind
13793	1	5128	7	10	NULL	0	NULL	 Bcl2	NULL	hypophosphorylated	binds	NULL	only			Bax	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_6_3509_s_128	9584191	(D) Only hypophosphorylated Bcl2 binds to Bax.	bind
13651	1	5129	6	NULL	NULL	NULL	NULL	p150	GP		bind					p21	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_9_3885_s_174	15082782	(D) p150 binds p21 promoter region in vivo.	bind
13794	1	5129	7	NULL	NULL	0	NULL	p150	NULL		binds	NULL				p21	NULL			promoter	NULL	in vivo	0	NULL	NULL	NULL	gw70_molcellbiol_24_9_3885_s_174	15082782	(D) p150 binds p21 promoter region in vivo.	bind
13652	1	5130	6	NULL	NULL	NULL	NULL	p68	GP		bind					CBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5363_s_218	10409727	(D) p68 binds to CBP.	bind
13795	1	5130	7	NULL	NULL	0	NULL	p68	NULL		binds	NULL				CBP	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_8_5363_s_218	10409727	(D) p68 binds to CBP.	bind
13748	1	5131	6	NULL	NULL	NULL	NULL	PAK2	GP		does not bind					TGF-betaR complex	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8878_s_119	14612425	(D) PAK2 does not bind the TGF-betaR complex.	bind
13796	1	5131	7	NULL	NULL	0	NULL	PAK2	NULL		does not bind	NULL				TGF-betaR complex	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8878_s_119	14612425	(D) PAK2 does not bind the TGF-betaR complex.	bind
13749	1	5132	6	NULL	NULL	NULL	NULL	aldolase	GP	parasite	bind		directly			actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_4_885_s_68	12718875	(D) Parasite aldolase binds directly to actin.	bind
13797	1	5132	7	NULL	NULL	0	NULL	aldolase	NULL	Parasite	binds	NULL	directly			actin	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_11_4_885_s_68	12718875	(D) Parasite aldolase binds directly to actin.	bind
13750	1	5133	6	NULL	NULL	NULL	NULL	Paxillin	GP		bind					PAG3	GP		COOH-terminal region		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_4_1315_s_146	10749932	(D) Paxillin binds to the COOH-terminal region of PAG3.	bind
13798	1	5133	7	NULL	NULL	0	NULL	Paxillin	NULL		binds to	NULL				PAG3	NULL		COOH-terminal 		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1315_s_146	10749932	(D) Paxillin binds to the COOH-terminal region of PAG3.	bind
13751	1	5134	6	NULL	NULL	NULL	NULL	Ptc2	GP	phosphorylated	bind					Rad53	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_3_827_s_114	12667463	(D) Phosphorylated Ptc2 binds to Rad53 irrespective of its phosphorylation state.	bind
13752	2	5134	6	NULL	NULL	NULL	NULL	statement 1	Process		irrespective of					Ptc2	GP	phosphorylation status of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_3_827_s_114	12667463	(D) Phosphorylated Ptc2 binds to Rad53 irrespective of its phosphorylation state.	bind
13799	1	5134	7	NULL	NULL	0	NULL	Ptc2	NULL	phosphorylated	binds to	NULL				Rad53	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_11_3_827_s_114	12667463	(D) Phosphorylated Ptc2 binds to Rad53 irrespective of its phosphorylation state.	bind
13800	2	5134	7	NULL	NULL	0	NULL	statement 1	NULL		irrespective of	NULL				Ptc2	NULL	 phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_3_827_s_114	12667463	(D) Phosphorylated Ptc2 binds to Rad53 irrespective of its phosphorylation state.	bind
13753	1	5135	6	NULL	NULL	NULL	NULL	BAF complex	Cell		bind					chromatin	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cell_95_5_625_s_92	9845365	(D) PIP2 enhances BAF complex binding to chromatin.	bind
13754	2	5135	6	NULL	NULL	NULL	NULL	PIP2	GP		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_95_5_625_s_92	9845365	(D) PIP2 enhances BAF complex binding to chromatin.	bind
13801	1	5135	7	NULL	NULL	0	NULL	BAF complex	NULL		binds	NULL				chromatin	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_95_5_625_s_92	9845365	(D) PIP2 enhances BAF complex binding to chromatin.	bind
13802	2	5135	7	NULL	NULL	0	NULL	PIP2	NULL		enhances	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_95_5_625_s_92	9845365	(D) PIP2 enhances BAF complex binding to chromatin.	bind
13755	1	5136	6	NULL	NULL	NULL	NULL	PLC 1	GP		bind					TrkB receptors	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_2_335_s_85	9728915	(D) PLC 1 binding to mutant TrkB receptors.	bind
13803	1	5136	7	NULL	NULL	0	NULL	PLC 1	NULL		bind	NULL				 TrkB receptor	NULL	mutant			NULL		0	NULL	NULL	NULL	gw60_neuron_21_2_335_s_85	9728915	(D) PLC 1 binding to mutant TrkB receptors.	bind
14093	1	5137	6	NULL	NULL	NULL	NULL	PP2A	GP		bind					ST	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_4_1298_s_147	15684382	(D) PP2A binding  to ST can be uncoupled from the ST-mediated transfer of PP2A onto AR.	bind
19010	3	5137	6	NULL	NULL	NULL	NULL	PP2A	GP		transfer to					AR	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_4_1298_s_147	15684382	(D) PP2A binding  to ST can be uncoupled from the ST-mediated transfer of PP2A onto AR.	bind
19011	4	5137	6	NULL	NULL	NULL	NULL	ST	GP		mediates					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_4_1298_s_147	15684382	(D) PP2A binding  to ST can be uncoupled from the ST-mediated transfer of PP2A onto AR.	bind
53052	5	5137	6	NULL	NULL	NULL	NULL	statement 1	Process		uncoupled by					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_4_1298_s_147	15684382	(D) PP2A binding  to ST can be uncoupled from the ST-mediated transfer of PP2A onto AR.	bind
13805	1	5137	7	NULL	NULL	0	NULL	PP2A	NULL		bind	NULL				ST	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_4_1298_s_147	15684382	(D) PP2A binding  to ST can be uncoupled from the ST-mediated transfer of PP2A onto AR.	bind
13811	2	5137	7	NULL	NULL	0	NULL	PP2A	NULL		transfer to	NULL				AR	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_4_1298_s_147	15684382	(D) PP2A binding  to ST can be uncoupled from the ST-mediated transfer of PP2A onto AR.	bind
13813	4	5137	7	10	NULL	0	NULL	statement 1	NULL		 uncoupled by	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_4_1298_s_147	15684382	(D) PP2A binding  to ST can be uncoupled from the ST-mediated transfer of PP2A onto AR.	bind
19030	3	5137	7	NULL	NULL	0	NULL	ST	NULL		mediates	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_4_1298_s_147	15684382	(D) PP2A binding  to ST can be uncoupled from the ST-mediated transfer of PP2A onto AR.	bind
13756	1	5138	6	NULL	NULL	NULL	NULL	Procaspase 3	GP	endogenous	bind					AKAP95	GP	endogenous			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_21_9469_s_151	16227597	(D) Procaspase 3 binds to AKAP95 at endogenous  protein levels.	bind
13816	1	5138	7	10	NULL	0	NULL	Procaspase 3	NULL	endogenous	binds	NULL				AKAP95	NULL	endogenous			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_21_9469_s_151	16227597	(D) Procaspase 3 binds to AKAP95 at endogenous  protein levels.	bind
13757	1	5139	6	NULL	NULL	NULL	NULL	Smurf2	GP		induces					receptor complex	GP	degradation of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_6_1365_s_177	11163210	(D) Proteasome and lysosome inhibitors block Smurf2-induced degradation of the receptor complex.	bind
13758	2	5139	6	NULL	NULL	NULL	NULL	proteasome inhibitors	Chemical		block					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_6_1365_s_177	11163210	(D) Proteasome and lysosome inhibitors block Smurf2-induced degradation of the receptor complex.	bind
13759	3	5139	6	NULL	NULL	NULL	NULL	lysosome inhibitors	GP		block					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_6_1365_s_177	11163210	(D) Proteasome and lysosome inhibitors block Smurf2-induced degradation of the receptor complex.	bind
13817	1	5139	7	NULL	NULL	0	NULL	Smurf2	NULL		induce	NULL				receptor complex	NULL	degradation of			NULL		0	NULL	NULL	NULL	gw60_molcell_6_6_1365_s_177	11163210	(D) Proteasome and lysosome inhibitors block Smurf2-induced degradation of the receptor complex.	bind
13818	2	5139	7	NULL	NULL	0	NULL	Proteasome inhibitor	NULL		block	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_6_6_1365_s_177	11163210	(D) Proteasome and lysosome inhibitors block Smurf2-induced degradation of the receptor complex.	bind
13819	3	5139	7	NULL	NULL	0	NULL	 lysosome inhibitor	NULL		block	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_6_6_1365_s_177	11163210	(D) Proteasome and lysosome inhibitors block Smurf2-induced degradation of the receptor complex.	bind
13760	1	5140	6	NULL	NULL	NULL	NULL	PU.1	GP		bind								CH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3729_s_184	11997509	(D) PU.1 binds to both the CH3 domain and the AT domain.	bind
13761	2	5140	6	NULL	NULL	NULL	NULL	PU.1	GP		bind								AT domain		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_11_3729_s_184	11997509	(D) PU.1 binds to both the CH3 domain and the AT domain.	bind
13820	1	5140	7	NULL	NULL	0	NULL	PU.1	NULL		binds	NULL					NULL		CH3 domain		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_11_3729_s_184	11997509	(D) PU.1 binds to both the CH3 domain and the AT domain.	bind
13821	2	5140	7	NULL	NULL	0	NULL	PU.1	NULL		binds	NULL					NULL		AT domain		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_11_3729_s_184	11997509	(D) PU.1 binds to both the CH3 domain and the AT domain.	bind
13762	1	5141	6	NULL	NULL	NULL	NULL	CDC48	GP	purified	bind					Ubi-GST	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_cell_107_5_667_s_240	11733065	(D) Purified CDC48  binds Ubi-GST but not GST in vitro.	bind
13763	2	5141	6	NULL	NULL	NULL	NULL	CDC48	GP	purified	does not bind					GST	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_cell_107_5_667_s_240	11733065	(D) Purified CDC48  binds Ubi-GST but not GST in vitro.	bind
13822	1	5141	7	NULL	NULL	0	NULL	CDC48	NULL	purified	binds	NULL				Ubi-GST	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_cell_107_5_667_s_240	11733065	(D) Purified CDC48  binds Ubi-GST but not GST in vitro.	bind
13823	2	5141	7	NULL	NULL	0	NULL	CDC48	NULL	purified	does not bind	NULL				GST	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_cell_107_5_667_s_240	11733065	(D) Purified CDC48  binds Ubi-GST but not GST in vitro.	bind
13764	1	5142	6	NULL	NULL	NULL	NULL	aldolase-His6	GP	purified;;recombinant;;Toxoplasma	bind		specifically			GST-MIC2t	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_4_885_s_117	12718875	(D) Purified recombinant  Toxoplasma aldolase-His6 (TgAld) also bound specifically to GST-MIC2t but not the W/A mutant.	bind
13765	2	5142	6	NULL	NULL	NULL	NULL	aldolase-His6	GP	purified;;recombinant;;Toxoplasma	does not bind					W/A 		mutant			NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_4_885_s_117	12718875	(D) Purified recombinant  Toxoplasma aldolase-His6 (TgAld) also bound specifically to GST-MIC2t but not the W/A mutant.	bind
13766	3	5142	6	NULL	NULL	NULL	NULL	TgAld	GP		is					Toxoplasma aldolase-His6	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_4_885_s_117	12718875	(D) Purified recombinant  Toxoplasma aldolase-His6 (TgAld) also bound specifically to GST-MIC2t but not the W/A mutant.	bind
13824	1	5142	7	10	NULL	0	NULL	aldolase-His6	NULL	purified;;recombinant;;Toxoplasma	bind	NULL	specifically			GST-MIC2t	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_4_885_s_117	12718875	(D) Purified recombinant  Toxoplasma aldolase-His6 (TgAld) also bound specifically to GST-MIC2t but not the W/A mutant.	bind
13828	2	5142	7	10	NULL	0	NULL	aldolase-His6	NULL	purified;;recombinant;;Toxoplasma	does not bind	NULL				W/A	NULL	mutant			NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_4_885_s_117	12718875	(D) Purified recombinant  Toxoplasma aldolase-His6 (TgAld) also bound specifically to GST-MIC2t but not the W/A mutant.	bind
13829	3	5142	7	NULL	NULL	0	NULL	TgAld	NULL		is	NULL				Toxoplasma aldolase-His6	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_4_885_s_117	12718875	(D) Purified recombinant  Toxoplasma aldolase-His6 (TgAld) also bound specifically to GST-MIC2t but not the W/A mutant.	bind
13767	1	5145	6	NULL	NULL	NULL	NULL	VDR	GP		bind					beta-catenin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_2_369_s_253	11470825	(D) Quantification of the amount of VDR bound to beta-catenin after 1alpha,25(OH)2D3 addition.	bind
44685	2	5145	6	NULL	NULL	NULL	NULL	1alpha,25(OH)2D3	Chemical	addition of	leads to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_2_369_s_253	11470825	(D) Quantification of the amount of VDR bound to beta-catenin after 1alpha,25(OH)2D3 addition.	bind
13832	1	5145	7	NULL	NULL	0	NULL	VDR	NULL		bind	NULL				beta-catenin	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_154_2_369_s_253	11470825	(D) Quantification of the amount of VDR bound to beta-catenin after 1alpha,25(OH)2D3 addition.	bind
13835	2	5145	7	10	NULL	0	NULL	statement 1	NULL		occurs after	NULL				1alpha,25(OH)2D3	NULL	addition of			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_2_369_s_253	11470825	(D) Quantification of the amount of VDR bound to beta-catenin after 1alpha,25(OH)2D3 addition.	bind
13768	1	5146	6	NULL	NULL	NULL	NULL	TOPBP1	GP		bind					Miz-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_3_509_s_113	12408820	(D) Quantitation of five independent immunoprecipitation experiments performed as in (C); the amount of TOPBP1 bound to Miz-1 in the absence of UV irradiation was arbitrarily set to one.	bind
13769	2	5146	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs in absence of					UV irradiation	MachineActivity				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_3_509_s_113	12408820	(D) Quantitation of five independent immunoprecipitation experiments performed as in (C); the amount of TOPBP1 bound to Miz-1 in the absence of UV irradiation was arbitrarily set to one.	bind
13836	1	5146	7	NULL	NULL	0	NULL	TOPBP1	NULL		bind	NULL				Miz-1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_3_509_s_113	12408820	(D) Quantitation of five independent immunoprecipitation experiments performed as in (C); the amount of TOPBP1 bound to Miz-1 in the absence of UV irradiation was arbitrarily set to one.	bind
19765	2	5146	7	NULL	NULL	0	NULL	statement 1	NULL		occurs in absence of	NULL				UV irradiation	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_10_3_509_s_113	12408820	(D) Quantitation of five independent immunoprecipitation experiments performed as in (C); the amount of TOPBP1 bound to Miz-1 in the absence of UV irradiation was arbitrarily set to one.	bind
14098	1	5147	6	NULL	NULL	NULL	NULL	InR	GP		bind					GST-IRS	GP	wild type	1108 - 516		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_166_2_213_s_177	15249583	(D) Quantitation of InR binding to  GST-IRS-1108 - 516 (WT) or a mutant GST-IRS-1108 - 516 in which serine 302 is mutated to alanine (S302A) after in vitro phosphorylation  by S6K2.	bind
14099	2	5147	6	NULL	NULL	NULL	NULL	InR	GP		bind					GST-IRS	GP	mutant	S302A 1108 - 516		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_166_2_213_s_177	15249583	(D) Quantitation of InR binding to  GST-IRS-1108 - 516 (WT) or a mutant GST-IRS-1108 - 516 in which serine 302 is mutated to alanine (S302A) after in vitro phosphorylation  by S6K2.	bind
14100	3	5147	6	NULL	NULL	0	NULL	S302A	NULL		is	NULL				serine 302 is mutated to alanine	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_166_2_213_s_177	15249583	(D) Quantitation of InR binding to  GST-IRS-1108 - 516 (WT) or a mutant GST-IRS-1108 - 516 in which serine 302 is mutated to alanine (S302A) after in vitro phosphorylation  by S6K2.	bind
14101	4	5147	6	NULL	NULL	0	NULL	S6K2	NULL		phosphorylates	NULL				GST-IRS	NULL		1108 - 516		NULL	in vitro	NULL	NULL	NULL	NULL	gw70_cellbiol_166_2_213_s_177	15249583	(D) Quantitation of InR binding to  GST-IRS-1108 - 516 (WT) or a mutant GST-IRS-1108 - 516 in which serine 302 is mutated to alanine (S302A) after in vitro phosphorylation  by S6K2.	bind
14102	5	5147	6	NULL	NULL	NULL	NULL	statement 4	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_166_2_213_s_177	15249583	(D) Quantitation of InR binding to  GST-IRS-1108 - 516 (WT) or a mutant GST-IRS-1108 - 516 in which serine 302 is mutated to alanine (S302A) after in vitro phosphorylation  by S6K2.	bind
13929	1	5147	7	NULL	NULL	0	NULL	InR	NULL		bind	NULL				GST-IRS	NULL	WT	1108 - 516		NULL		0	NULL	NULL	NULL	gw70_cellbiol_166_2_213_s_177	15249583	(D) Quantitation of InR binding to  GST-IRS-1108 - 516 (WT) or a mutant GST-IRS-1108 - 516 in which serine 302 is mutated to alanine (S302A) after in vitro phosphorylation  by S6K2.	bind
13932	2	5147	7	NULL	NULL	0	NULL	S6K2	NULL		phosphorylates	NULL				 GST-IRS	NULL	mutant	1108 - 516 S302A		NULL	in vitro	0	NULL	NULL	NULL	gw70_cellbiol_166_2_213_s_177	15249583	(D) Quantitation of InR binding to  GST-IRS-1108 - 516 (WT) or a mutant GST-IRS-1108 - 516 in which serine 302 is mutated to alanine (S302A) after in vitro phosphorylation  by S6K2.	bind
13933	3	5147	7	NULL	NULL	0	NULL	InR	NULL		bind	NULL				GST-IRS	NULL	mutant	1108 - 516 S302A		NULL		0	NULL	NULL	NULL	gw70_cellbiol_166_2_213_s_177	15249583	(D) Quantitation of InR binding to  GST-IRS-1108 - 516 (WT) or a mutant GST-IRS-1108 - 516 in which serine 302 is mutated to alanine (S302A) after in vitro phosphorylation  by S6K2.	bind
13934	4	5147	7	NULL	NULL	0	NULL	statement 3	NULL		occurs after	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_166_2_213_s_177	15249583	(D) Quantitation of InR binding to  GST-IRS-1108 - 516 (WT) or a mutant GST-IRS-1108 - 516 in which serine 302 is mutated to alanine (S302A) after in vitro phosphorylation  by S6K2.	bind
53053	5	5147	7	10	NULL	0	NULL	S302A	NULL		is	NULL				serine 302 is mutated to alanine	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_166_2_213_s_177	15249583	(D) Quantitation of InR binding to  GST-IRS-1108 - 516 (WT) or a mutant GST-IRS-1108 - 516 in which serine 302 is mutated to alanine (S302A) after in vitro phosphorylation  by S6K2.	bind
13770	1	5148	6	NULL	NULL	NULL	NULL	Rad32	GP		bind			D25A		Rad50	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_15_5186_s_185	12861005	(D) Rad32-D25A binds to Rad50 in immunoprecipitation assay.	bind
13935	1	5148	7	NULL	NULL	0	NULL	Rad32	NULL		binds	NULL		D25A		Rad50	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_15_5186_s_185	12861005	(D) Rad32-D25A binds to Rad50 in immunoprecipitation assay.	bind
13771	1	5152	6	NULL	NULL	NULL	NULL	Gal4-Knirps chimera	GP		mediates			202-358		repression	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7247_s_258	10982842	(D) Repression mediated by the Gal4-Knirps (202-358) chimera, a protein that contains the dCtBP interaction motif.	bind
13775	2	5152	6	NULL	NULL	NULL	NULL	Gal4-Knirps chimera	GP		contain			202-358					dCtBP interaction motif		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7247_s_258	10982842	(D) Repression mediated by the Gal4-Knirps (202-358) chimera, a protein that contains the dCtBP interaction motif.	bind
13947	1	5152	7	NULL	NULL	0	NULL	chimera Gal4-Knirps	NULL		contains	NULL		202-358			NULL		dCtBP interaction motif		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7247_s_258	10982842	(D) Repression mediated by the Gal4-Knirps (202-358) chimera, a protein that contains the dCtBP interaction motif.	bind
13948	2	5152	7	NULL	NULL	0	NULL	chimera Gal4-Knirps	NULL		mediates	NULL		202-358		repression	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7247_s_258	10982842	(D) Repression mediated by the Gal4-Knirps (202-358) chimera, a protein that contains the dCtBP interaction motif.	bind
13776	1	5153	6	NULL	NULL	NULL	NULL	BCS1	GP		bind					OMV	Organism				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_7_2239_s_283	12640110	(D) Residues 87 to 126 of BCS1 increase binding  to OMV.	bind
13777	2	5153	6	NULL	NULL	NULL	NULL	BCS1	GP		increase			residues 87 to 126		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_7_2239_s_283	12640110	(D) Residues 87 to 126 of BCS1 increase binding  to OMV.	bind
13949	1	5153	7	NULL	NULL	0	NULL	BCS1	NULL		bind	NULL				OMV	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_7_2239_s_283	12640110	(D) Residues 87 to 126 of BCS1 increase binding  to OMV.	bind
13950	2	5153	7	NULL	NULL	0	NULL	BCS1	NULL		increase	NULL		Residues 87 to 126		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_7_2239_s_283	12640110	(D) Residues 87 to 126 of BCS1 increase binding  to OMV.	bind
13778	1	5156	6	NULL	NULL	NULL	NULL	CSL	GP		bind					Caco-2 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_10_5282_s_240	10496907	(D) Saturability of CSL binding to Caco-2 cells.	bind
13951	1	5156	7	NULL	NULL	0	NULL	CSL	NULL		bind	NULL				Caco-2 cells	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_67_10_5282_s_240	10496907	(D) Saturability of CSL binding to Caco-2 cells.	bind
13779	1	5158	6	NULL	NULL	NULL	NULL	Sem-AP	GP		bind					NP	GP	mutants			NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_5_1093_s_73	9856464	(D) Sem-AP binding to NP mutants.	bind
13952	1	5158	7	NULL	NULL	0	NULL	Sem-AP	NULL		bind	NULL				 NP	NULL	mutant			NULL		0	NULL	NULL	NULL	gw60_neuron_21_5_1093_s_73	9856464	(D) Sem-AP binding to NP mutants.	bind
13780	1	5161	6	NULL	NULL	NULL	NULL	Skp2	GP		bind		directly			Smad4	GP	cancer mutants			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_17_7524_s_129	15314162	(D) Skp2 binds to Smad4 cancer mutants directly in  vitro.	bind
13955	1	5161	7	NULL	NULL	0	NULL	Skp2 	NULL		binds	NULL	directly			Smad4	NULL	cancer mutant			NULL	in vitro	0	NULL	NULL	NULL	gw70_molcellbiol_24_17_7524_s_129	15314162	(D) Skp2 binds to Smad4 cancer mutants directly in  vitro.	bind
13781	1	5162	6	NULL	NULL	NULL	NULL	Smurf2	GP		increases					IFN	GP	inhibitory effect of 			NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_6_1365_s_258	11163210	(D) Smurf2 increases IFN  inhibitory effect.	bind
13956	1	5162	7	NULL	NULL	0	NULL	Smurf2 	NULL		increase	NULL				IFN	NULL	inhibitory effect of			NULL		0	NULL	NULL	NULL	gw60_molcell_6_6_1365_s_258	11163210	(D) Smurf2 increases IFN  inhibitory effect.	bind
13782	1	5163	6	NULL	NULL	NULL	NULL	CRM1	GP		bind					Nup214	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_18_6772_s_317	16943420	(D) Solid-phase binding  of CRM1 to Nup214 was analyzed in the absence or presence of RanGTPgammaS, RanGDP, or NES peptide, as indicated.	bind
13957	1	5163	7	NULL	NULL	0	NULL	CRM1	NULL		bind	NULL				Nup214	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_18_6772_s_317	16943420	(D) Solid-phase binding  of CRM1 to Nup214 was analyzed in the absence or presence of RanGTPgammaS, RanGDP, or NES peptide, as indicated.	bind
13783	2	5164	6	NULL	NULL	NULL	NULL	statement 1	Process		bind		specifically			hsp27	GP			EcRE	NULL		NULL	NULL	NULL	NULL	gw60_insectbiochemmolbiol_28_11_849_s_166	9818386	(d) Specific binding of hsp27 EcRE to the EcR complex that had been pretreated with  -protein phosphatase.	bind
13784	1	5164	6	NULL	NULL	NULL	NULL	EcR complex	GP		pre-treated with					protein phosphatase	GP				NULL		NULL	NULL	NULL	NULL	gw60_insectbiochemmolbiol_28_11_849_s_166	9818386	(d) Specific binding of hsp27 EcRE to the EcR complex that had been pretreated with  -protein phosphatase.	bind
13958	1	5164	7	NULL	NULL	0	NULL	hsp27 	NULL		bind	NULL	specifically		EcRE	EcR complex 	NULL				NULL		NULL	NULL	NULL	NULL	gw60_insectbiochemmolbiol_28_11_849_s_166	9818386	(d) Specific binding of hsp27 EcRE to the EcR complex that had been pretreated with  -protein phosphatase.	bind
13959	2	5164	7	NULL	NULL	0	NULL	EcR complex	NULL		pretreated with	NULL				protein phosphatase	NULL				NULL		NULL	NULL	NULL	NULL	gw60_insectbiochemmolbiol_28_11_849_s_166	9818386	(d) Specific binding of hsp27 EcRE to the EcR complex that had been pretreated with  -protein phosphatase.	bind
13785	1	5165	6	NULL	NULL	NULL	NULL	NFATc	GP		bind		specifically	DBD		SE RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_298_4_486_s_73	12408978	(D) Specific binding of NFATc DBD to SE RNA #1.	bind
13960	1	5165	7	10	NULL	0	NULL	NFATc 	NULL		bind	NULL	specifically	DBD		SE RNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_298_4_486_s_73	12408978	(D) Specific binding of NFATc DBD to SE RNA #1.	bind
13786	1	5166	6	NULL	NULL	NULL	NULL	HMG-I	GP		bind					HPV18 	Organism	wt			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_7_2329_s_184	12640118	(D) Specific competition of the AP1 and HMG-I(Y) binding  on the HPV18 wt probe.	bind
13787	2	5166	6	NULL	NULL	NULL	NULL	AP1	GP		bind					HPV18	Organism	wt			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_7_2329_s_184	12640118	(D) Specific competition of the AP1 and HMG-I(Y) binding  on the HPV18 wt probe.	bind
13788	3	5166	6	NULL	NULL	NULL	NULL	statement 1	Process		competes with		specifically			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_7_2329_s_184	12640118	(D) Specific competition of the AP1 and HMG-I(Y) binding  on the HPV18 wt probe.	bind
13961	1	5166	7	NULL	NULL	0	NULL	AP1	NULL		bind	NULL				HPV18	NULL	wt			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_7_2329_s_184	12640118	(D) Specific competition of the AP1 and HMG-I(Y) binding  on the HPV18 wt probe.	bind
13962	2	5166	7	NULL	NULL	0	NULL	HMG-I	NULL		bind	NULL				HPV18	NULL	wt			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_7_2329_s_184	12640118	(D) Specific competition of the AP1 and HMG-I(Y) binding  on the HPV18 wt probe.	bind
13974	3	5166	7	NULL	NULL	0	NULL	statement 1	NULL		compete with	NULL	specifically			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_7_2329_s_184	12640118	(D) Specific competition of the AP1 and HMG-I(Y) binding  on the HPV18 wt probe.	bind
19012	1	5167	6	NULL	NULL	NULL	NULL	AKAP79	GP		bind		specifically			PSD-95	GP	mutant	SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_neuron_27_1_107_s_175	10939335	(D) Specificity of AKAP79 binding to the SH3 domain binding was tested in pulldown experiments using SH3 domain mutants of PSD-95.	bind
13976	1	5167	7	NULL	NULL	0	NULL	AKAP79	NULL		bind	NULL	specifically			PSD-95	NULL	mutant	SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_neuron_27_1_107_s_175	10939335	(D) Specificity of AKAP79 binding to the SH3 domain binding was tested in pulldown experiments using SH3 domain mutants of PSD-95.	bind
13804	1	5168	6	NULL	NULL	NULL	NULL	NAD+	Chemical		bind		specifically			RIBEYE	GP		B domain		NULL		NULL	NULL	NULL	NULL	gw60_neuron_28_3_857_s_260	11163272	(D) Specificity of NAD+ binding to the B domain of RIBEYE.	bind
13977	1	5168	7	NULL	NULL	0	NULL	NAD+	NULL		bind	NULL	specifically			RIBEYE	NULL		B domain		NULL		0	NULL	NULL	NULL	gw60_neuron_28_3_857_s_260	11163272	(D) Specificity of NAD+ binding to the B domain of RIBEYE.	bind
13806	1	5169	6	NULL	NULL	NULL	NULL	p53	GP		bind					Apaf1	GP			promoter	NULL	p53+/+ neurons treated with camptothecin	NULL	NULL	NULL	NULL	gw60_cellbiol_155_2_207_s_94	11591730	(D) Specificity of p53 binding activity to the Apaf1 promoter was examined in p53+/+ and p53-/- neurons treated with camptothecin.	bind
13807	2	5169	6	NULL	NULL	NULL	NULL	p53	GP		bind					Apaf1	GP			promoter	NULL	p53-/- neurons treated with camptothecin	NULL	NULL	NULL	NULL	gw60_cellbiol_155_2_207_s_94	11591730	(D) Specificity of p53 binding activity to the Apaf1 promoter was examined in p53+/+ and p53-/- neurons treated with camptothecin.	bind
13978	1	5169	7	NULL	NULL	0	NULL	p53	NULL		bind	NULL				Apaf1	NULL			promoter	NULL	p53+/+ neurons treated with camptothecin	NULL	NULL	NULL	NULL	gw60_cellbiol_155_2_207_s_94	11591730	(D) Specificity of p53 binding activity to the Apaf1 promoter was examined in p53+/+ and p53-/- neurons treated with camptothecin.	bind
13979	2	5169	7	NULL	NULL	0	NULL	p53	NULL		bind	NULL				Apaf1	NULL			promoter	NULL	p53-/- neurons treated with camptothecin	NULL	NULL	NULL	NULL	gw60_cellbiol_155_2_207_s_94	11591730	(D) Specificity of p53 binding activity to the Apaf1 promoter was examined in p53+/+ and p53-/- neurons treated with camptothecin.	bind
13808	1	5171	6	NULL	NULL	NULL	NULL	MMP-2	GP		cleaves					Ln-5	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_161_1_197_s_209	12695504	(D) Stimulated migration of  MMP-2 cleaved Ln-5 depends on EGFR. MCF10A cells were allowed to migrate on Transwell  membranes, which were coated with either uncleaved (top panels; -MMP-2) or MMP-2-cleaved  Ln-5 (bottom panels; +MMP-2).	bind
13809	2	5171	6	NULL	NULL	NULL	NULL	Ln-5	GP	migration of;;MMP-2 cleaved	is dependent on					EGFR	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_161_1_197_s_209	12695504	(D) Stimulated migration of  MMP-2 cleaved Ln-5 depends on EGFR. MCF10A cells were allowed to migrate on Transwell  membranes, which were coated with either uncleaved (top panels; -MMP-2) or MMP-2-cleaved  Ln-5 (bottom panels; +MMP-2).	bind
14050	1	5171	7	NULL	NULL	0	NULL	MMP-2 	NULL		cleaves	NULL				Ln-5	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_161_1_197_s_209	12695504	(D) Stimulated migration of  MMP-2 cleaved Ln-5 depends on EGFR. MCF10A cells were allowed to migrate on Transwell  membranes, which were coated with either uncleaved (top panels; -MMP-2) or MMP-2-cleaved  Ln-5 (bottom panels; +MMP-2).	bind
14051	2	5171	7	10	NULL	0	NULL	Ln-5	NULL	migration of;;MMP-2 cleaved	depends on	NULL				EGFR	NULL				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_161_1_197_s_209	12695504	(D) Stimulated migration of  MMP-2 cleaved Ln-5 depends on EGFR. MCF10A cells were allowed to migrate on Transwell  membranes, which were coated with either uncleaved (top panels; -MMP-2) or MMP-2-cleaved  Ln-5 (bottom panels; +MMP-2).	bind
13810	1	5172	6	NULL	NULL	NULL	NULL	GTP S 	Chemical		bind					Rab5	GP				NULL	early endosomes	NULL	NULL	NULL	NULL	gw60_cell_90_6_1149_s_172	9323142	(d) Stimulation of [35]GTP S  binding to Rab5 on early endosomes by the Rabaptin-5 - p60 complex.	bind
13812	2	5172	6	NULL	NULL	NULL	NULL	Rabaptin-5 - p60 complex	GP		stimulates					statement 1	Process				NULL	early endosomes	NULL	NULL	NULL	NULL	gw60_cell_90_6_1149_s_172	9323142	(d) Stimulation of [35]GTP S  binding to Rab5 on early endosomes by the Rabaptin-5 - p60 complex.	bind
14052	1	5172	7	10	NULL	0	NULL	GTP S 	NULL		bind	NULL				Rab5	NULL				NULL	early endosomes	NULL	NULL	NULL	NULL	gw60_cell_90_6_1149_s_172	9323142	(d) Stimulation of [35]GTP S  binding to Rab5 on early endosomes by the Rabaptin-5 - p60 complex.	bind
14053	2	5172	7	10	NULL	0	NULL	Rabaptin-5 - p60 complex	NULL		stimulate	NULL				statement 1	NULL				NULL	early endosomes	NULL	NULL	NULL	NULL	gw60_cell_90_6_1149_s_172	9323142	(d) Stimulation of [35]GTP S  binding to Rab5 on early endosomes by the Rabaptin-5 - p60 complex.	bind
13814	1	5173	6	NULL	NULL	NULL	NULL	SNARE proteins	GP		bind					MYC-Sec1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_146_2_333_s_157	10427089	(D) Stoichiometry of SNARE proteins bound to MYC-Sec1p.	bind
14054	1	5173	7	NULL	NULL	0	NULL	SNARE protein	NULL		bind	NULL				MYC-Sec1p	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_146_2_333_s_157	10427089	(D) Stoichiometry of SNARE proteins bound to MYC-Sec1p.	bind
13815	1	5174	6	NULL	NULL	NULL	NULL	SA	Chemical		bind					EL229C-B					NULL		NULL	NULL	NULL	NULL	gw60_cell_107_2_223_s_81	11672529	(D) Stopped-flow kinetics of SA binding to  EL229C-B.	bind
14055	1	5174	7	NULL	NULL	0	NULL	SA	NULL		bind	NULL				EL229C-B	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_107_2_223_s_81	11672529	(D) Stopped-flow kinetics of SA binding to  EL229C-B.	bind
13963	1	5175	6	NULL	NULL	NULL	NULL	Stx	GP		bind					glomeruli 	OrganismPart	immature;;outer cortex			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_1_612_s_63	15618202	(D) Stx binding to immature glomeruli (IG) of outer cortex.	bind
19013	2	5175	6	NULL	NULL	NULL	NULL	IG	OrganismPart		is					immature glomeruli	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_1_612_s_63	15618202	(D) Stx binding to immature glomeruli (IG) of outer cortex.	bind
14056	1	5175	7	10	NULL	0	NULL	Stx	NULL		bind	NULL				 glomeruli	NULL	immature;;outer cortex			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_1_612_s_63	15618202	(D) Stx binding to immature glomeruli (IG) of outer cortex.	bind
14057	2	5175	7	NULL	NULL	0	NULL	IG	NULL		is	NULL				 immature glomeruli 	NULL				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_1_612_s_63	15618202	(D) Stx binding to immature glomeruli (IG) of outer cortex.	bind
13964	1	5176	6	NULL	NULL	NULL	NULL	Sec15p	GP		bind					Sec2p constructs	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_6_2757_s_228	16611746	(D) Summary of Sec15p and Ypt32p binding to Sec2p  constructs.	bind
13965	2	5176	6	NULL	NULL	NULL	NULL	Ypt32p	GP		bind					Sec2p constructs	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_6_2757_s_228	16611746	(D) Summary of Sec15p and Ypt32p binding to Sec2p  constructs.	bind
14058	1	5176	7	NULL	NULL	0	NULL	Sec15p	NULL		bind	NULL				Sec2p constructs	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_6_2757_s_228	16611746	(D) Summary of Sec15p and Ypt32p binding to Sec2p  constructs.	bind
14059	2	5176	7	NULL	NULL	0	NULL	Ypt32p	NULL		bind	NULL				Sec2p constructs	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_6_2757_s_228	16611746	(D) Summary of Sec15p and Ypt32p binding to Sec2p  constructs.	bind
13966	1	5178	6	NULL	NULL	NULL	NULL	caspase-7	GP	active	bind			catalytic groove		XIAP fragment					NULL		NULL	NULL	NULL	NULL	gw60_cell_107_3_399_s_56	11701129	(D) Surface representation of the catalytic groove  in the active caspase-7 bound with an  XIAP fragment.	bind
14060	1	5178	7	10	NULL	0	NULL	caspase-7	NULL	active	bind	NULL		catalytic groove		XIAP fragment	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_3_399_s_56	11701129	(D) Surface representation of the catalytic groove  in the active caspase-7 bound with an  XIAP fragment.	bind
13967	1	5179	6	NULL	NULL	NULL	NULL	Swi/nf	GP		displace					nucleosomes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_7_2078_s_392	11884596	(D) Swi/nf and SAGA displace nucleosomes, allowing binding of Ste12 and Tec1 to their sites.	bind
13968	2	5179	6	NULL	NULL	NULL	NULL	SAGA	GP		displace					nucleosomes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_7_2078_s_392	11884596	(D) Swi/nf and SAGA displace nucleosomes, allowing binding of Ste12 and Tec1 to their sites.	bind
13969	3	5179	6	NULL	NULL	NULL	NULL	Ste12	GP		bind									site	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_7_2078_s_392	11884596	(D) Swi/nf and SAGA displace nucleosomes, allowing binding of Ste12 and Tec1 to their sites.	bind
13970	4	5179	6	NULL	NULL	NULL	NULL	Tec1	GP		bind									site	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_7_2078_s_392	11884596	(D) Swi/nf and SAGA displace nucleosomes, allowing binding of Ste12 and Tec1 to their sites.	bind
13971	5	5179	6	NULL	NULL	NULL	NULL	statement 1	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_7_2078_s_392	11884596	(D) Swi/nf and SAGA displace nucleosomes, allowing binding of Ste12 and Tec1 to their sites.	bind
13972	6	5179	6	NULL	NULL	NULL	NULL	statement 1	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_7_2078_s_392	11884596	(D) Swi/nf and SAGA displace nucleosomes, allowing binding of Ste12 and Tec1 to their sites.	bind
13973	7	5179	6	NULL	NULL	NULL	NULL	statement 2	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_7_2078_s_392	11884596	(D) Swi/nf and SAGA displace nucleosomes, allowing binding of Ste12 and Tec1 to their sites.	bind
13975	8	5179	6	NULL	NULL	NULL	NULL	statement 2	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_7_2078_s_392	11884596	(D) Swi/nf and SAGA displace nucleosomes, allowing binding of Ste12 and Tec1 to their sites.	bind
14061	1	5179	7	NULL	NULL	0	NULL	Swi/nf 	NULL		displace	NULL				nucleosomes	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_7_2078_s_392	11884596	(D) Swi/nf and SAGA displace nucleosomes, allowing binding of Ste12 and Tec1 to their sites.	bind
14062	2	5179	7	NULL	NULL	0	NULL	SAGA	NULL		displace	NULL				nucleosomes	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_7_2078_s_392	11884596	(D) Swi/nf and SAGA displace nucleosomes, allowing binding of Ste12 and Tec1 to their sites.	bind
14063	3	5179	7	10	NULL	0	NULL	Ste12			bind					Swi/nf 					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_7_2078_s_392	11884596	(D) Swi/nf and SAGA displace nucleosomes, allowing binding of Ste12 and Tec1 to their sites.	bind
14064	4	5179	7	10	NULL	0	NULL	Ste12			bind					SAGA					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_7_2078_s_392	11884596	(D) Swi/nf and SAGA displace nucleosomes, allowing binding of Ste12 and Tec1 to their sites.	bind
14065	5	5179	7	NULL	NULL	0	NULL	statement 1	NULL		allows	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_7_2078_s_392	11884596	(D) Swi/nf and SAGA displace nucleosomes, allowing binding of Ste12 and Tec1 to their sites.	bind
14066	6	5179	7	NULL	NULL	0	NULL	statement 2	NULL		allows	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_7_2078_s_392	11884596	(D) Swi/nf and SAGA displace nucleosomes, allowing binding of Ste12 and Tec1 to their sites.	bind
14067	7	5179	7	NULL	NULL	0	NULL	Tec1	NULL		bind	NULL				Swi/nf 	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_7_2078_s_392	11884596	(D) Swi/nf and SAGA displace nucleosomes, allowing binding of Ste12 and Tec1 to their sites.	bind
14068	8	5179	7	NULL	NULL	0	NULL	Tec1	NULL		bind	NULL				SAGA	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_7_2078_s_392	11884596	(D) Swi/nf and SAGA displace nucleosomes, allowing binding of Ste12 and Tec1 to their sites.	bind
14069	9	5179	7	NULL	NULL	0	NULL	statement 1	NULL		allows	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_7_2078_s_392	11884596	(D) Swi/nf and SAGA displace nucleosomes, allowing binding of Ste12 and Tec1 to their sites.	bind
14070	10	5179	7	NULL	NULL	0	NULL	statement 2	NULL		allows	NULL				statement 8	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_7_2078_s_392	11884596	(D) Swi/nf and SAGA displace nucleosomes, allowing binding of Ste12 and Tec1 to their sites.	bind
13980	1	5180	6	NULL	NULL	NULL	NULL	SWI/SNF	GP		bind					HO	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4095_s_38	16705163	(D) SWI/SNF binding to  HO is restored in a  gcn5 sin3 strain.	bind
13981	2	5180	6	NULL	NULL	NULL	NULL	statement 1	Process		restored in					gcn5 sin3 strain	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4095_s_38	16705163	(D) SWI/SNF binding to  HO is restored in a  gcn5 sin3 strain.	bind
14071	1	5180	7	NULL	NULL	0	NULL	SWI/SNF	NULL		bind	NULL				HO	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_11_4095_s_38	16705163	(D) SWI/SNF binding to  HO is restored in a  gcn5 sin3 strain.	bind
14072	2	5180	7	NULL	NULL	0	NULL	statement 1	NULL		is restored in	NULL				 gcn5 sin3 strain	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_11_4095_s_38	16705163	(D) SWI/SNF binding to  HO is restored in a  gcn5 sin3 strain.	bind
13982	1	5181	6	NULL	NULL	NULL	NULL	Syntaxin	GP		bind					syt IX	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4755_s_213	16093350	(D) Syntaxin bound to  syt IX (C) was quantified by densitometry.	bind
14073	1	5181	7	NULL	NULL	0	NULL	Syntaxin	NULL		bind	NULL				syt IX	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4755_s_213	16093350	(D) Syntaxin bound to  syt IX (C) was quantified by densitometry.	bind
13983	1	5182	6	NULL	NULL	NULL	NULL	TCR	GP		bind					Nck	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_109_7_901_s_139	12110186	(D) Temperature dependence of TCR binding to Nck.	bind
13984	2	5182	6	NULL	NULL	NULL	NULL	statement 1	Process		is dependent on					temperature	AbstractConcept				NULL		NULL	NULL	NULL	NULL	gw60_cell_109_7_901_s_139	12110186	(D) Temperature dependence of TCR binding to Nck.	bind
14074	1	5182	7	NULL	NULL	0	NULL	TCR	NULL		bind	NULL				Nck	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_109_7_901_s_139	12110186	(D) Temperature dependence of TCR binding to Nck.	bind
14075	2	5182	7	NULL	NULL	0	NULL	statement 1	NULL		depends on	NULL				temperature	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_109_7_901_s_139	12110186	(D) Temperature dependence of TCR binding to Nck.	bind
13985	1	5183	6	NULL	NULL	NULL	NULL	annexin V	GP		bind					PKC	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_5_1151_s_190	12769841	(D) The  5 integrin cytoplasmic domain inhibits binding of annexin V to PKC.	bind
13986	2	5183	6	NULL	NULL	NULL	NULL	5 integrin	GP		inhibits			cytoplasmic domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_5_1151_s_190	12769841	(D) The  5 integrin cytoplasmic domain inhibits binding of annexin V to PKC.	bind
14076	1	5183	7	NULL	NULL	0	NULL	annexin V	NULL		bind	NULL				PKC	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_11_5_1151_s_190	12769841	(D) The  5 integrin cytoplasmic domain inhibits binding of annexin V to PKC.	bind
14077	2	5183	7	NULL	NULL	0	NULL	5 integrin	NULL		inhibits	NULL		cytoplasmic domain		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_11_5_1151_s_190	12769841	(D) The  5 integrin cytoplasmic domain inhibits binding of annexin V to PKC.	bind
13987	1	5184	6	NULL	NULL	NULL	NULL	semaphorin	GP		bind					NP/Plex 1 complexes	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_99_1_59_s_89	10520994	(D) The  affinity of semaphorin binding to various NP/Plex 1 complexes.	bind
14078	1	5184	7	NULL	NULL	0	NULL	semaphorin	NULL		bind	NULL				NP/Plex 1 complex 	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_99_1_59_s_89	10520994	(D) The  affinity of semaphorin binding to various NP/Plex 1 complexes.	bind
13988	1	5185	6	NULL	NULL	NULL	NULL	BRG1 proteins	GP	mutant	does not bind					pRB	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_3_1188_s_293	14729964	(D) The  mutant BRG1 proteins that do not bind pRB are capable of inducing formation of flat  cells.	bind
13989	2	5185	6	NULL	NULL	NULL	NULL	BRG1 proteins	GP	mutant	induce					flat cells	Cell	formation of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_3_1188_s_293	14729964	(D) The  mutant BRG1 proteins that do not bind pRB are capable of inducing formation of flat  cells.	bind
14079	1	5185	7	10	NULL	0	NULL	BRG1 protein	NULL	mutant	does not bind	NULL				pRB	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_3_1188_s_293	14729964	(D) The  mutant BRG1 proteins that do not bind pRB are capable of inducing formation of flat  cells.	bind
14080	2	5185	7	10	NULL	0	NULL	BRG1 protein	NULL	mutant	induce	NULL				flat cells	NULL	formation of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_3_1188_s_293	14729964	(D) The  mutant BRG1 proteins that do not bind pRB are capable of inducing formation of flat  cells.	bind
13990	1	5186	6	NULL	NULL	NULL	NULL	eIF5	GP		bind					NIP1	GP		NTD		NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9437_s_261	15485912	(D) The  NIP1-Box6 mutation diminishes binding of eIF5 and eIF2 to the NIP1-NTD in vivo.	bind
13991	2	5186	6	NULL	NULL	NULL	NULL	eIF2	GP		bind					NIP1	GP		NTD		NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9437_s_261	15485912	(D) The  NIP1-Box6 mutation diminishes binding of eIF5 and eIF2 to the NIP1-NTD in vivo.	bind
13992	3	5186	6	NULL	NULL	NULL	NULL	NIP1	GP	mutant	diminishes			Box6		statement 1	Process				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9437_s_261	15485912	(D) The  NIP1-Box6 mutation diminishes binding of eIF5 and eIF2 to the NIP1-NTD in vivo.	bind
13993	4	5186	6	NULL	NULL	NULL	NULL	NIP1	GP	mutant	diminishes			Box6		statement 2	Process				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9437_s_261	15485912	(D) The  NIP1-Box6 mutation diminishes binding of eIF5 and eIF2 to the NIP1-NTD in vivo.	bind
14081	1	5186	7	NULL	NULL	0	NULL	 eIF5	NULL		bind	NULL				NIP1	NULL		NTD		NULL	in vivo	0	NULL	NULL	NULL	gw70_molcellbiol_24_21_9437_s_261	15485912	(D) The  NIP1-Box6 mutation diminishes binding of eIF5 and eIF2 to the NIP1-NTD in vivo.	bind
14082	2	5186	7	NULL	NULL	0	NULL	eIF2	NULL		bind	NULL				NIP1	NULL		NTD		NULL	in vivo	0	NULL	NULL	NULL	gw70_molcellbiol_24_21_9437_s_261	15485912	(D) The  NIP1-Box6 mutation diminishes binding of eIF5 and eIF2 to the NIP1-NTD in vivo.	bind
14083	3	5186	7	10	NULL	0	NULL	NIP1	NULL	mutant	diminishes	NULL		Box6		statement 1	NULL				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9437_s_261	15485912	(D) The  NIP1-Box6 mutation diminishes binding of eIF5 and eIF2 to the NIP1-NTD in vivo.	bind
14084	4	5186	7	10	NULL	0	NULL	NIP1	NULL	mutant	diminishes	NULL		Box6		statement 2	NULL				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9437_s_261	15485912	(D) The  NIP1-Box6 mutation diminishes binding of eIF5 and eIF2 to the NIP1-NTD in vivo.	bind
13994	1	5187	6	NULL	NULL	NULL	NULL	38 kDa protein	GP		bind					GST - BRCA1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_88_2_265_s_134	9008167	(D) The 38 kDa protein bound to GST - BRCA1  #4 is a product of the human cell extract and can be  reimmunoprecipitated with Rad51 antiserum.	bind
13995	2	5187	6	NULL	NULL	NULL	NULL	38 kDa protein	GP		is a product of					cell extract	OrganismPart	human			NULL		NULL	NULL	NULL	NULL	gw60_cell_88_2_265_s_134	9008167	(D) The 38 kDa protein bound to GST - BRCA1  #4 is a product of the human cell extract and can be  reimmunoprecipitated with Rad51 antiserum.	bind
13996	3	5187	6	NULL	NULL	NULL	NULL	38 kDa protein	GP		reimmunoprecipitates with					Rad51 antiserum	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_88_2_265_s_134	9008167	(D) The 38 kDa protein bound to GST - BRCA1  #4 is a product of the human cell extract and can be  reimmunoprecipitated with Rad51 antiserum.	bind
14103	1	5187	7	10	NULL	0	NULL	38 kDa protein	NULL		bind	NULL				GST - BRCA1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cell_88_2_265_s_134	9008167	(D) The 38 kDa protein bound to GST - BRCA1  #4 is a product of the human cell extract and can be  reimmunoprecipitated with Rad51 antiserum.	bind
53056	2	5187	7	10	NULL	0	NULL	38 kDa protein	NULL		is a product of	NULL				cell extract	NULL	human			NULL		0	NULL	NULL	NULL	gw60_cell_88_2_265_s_134	9008167	(D) The 38 kDa protein bound to GST - BRCA1  #4 is a product of the human cell extract and can be  reimmunoprecipitated with Rad51 antiserum.	bind
53057	2	5187	7	10	NULL	0	NULL	38 kDa protein	NULL		reimmunoprecipitates with\t	NULL				Rad51 antiserum	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_88_2_265_s_134	9008167	(D) The 38 kDa protein bound to GST - BRCA1  #4 is a product of the human cell extract and can be  reimmunoprecipitated with Rad51 antiserum.	bind
13997	1	5188	6	NULL	NULL	NULL	NULL	Arp2/3	GP		bind					GST-VCA	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_150_6_1299_s_78	10995436	(D) The ability of HT-WG (2 muM) to inhibit the binding of Arp2/3 (0.1 muM) to GST-VCA (0.2 muM) was tested in the presence of GTPgammaS-loaded Cdc42 (5 muM) or PI(4,5)P2-containing vesicles (100 muM; PI(4,5)P2/PI/PC = 10:45:45).	bind
13998	2	5188	6	NULL	NULL	NULL	NULL	HT-WG	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_150_6_1299_s_78	10995436	(D) The ability of HT-WG (2 muM) to inhibit the binding of Arp2/3 (0.1 muM) to GST-VCA (0.2 muM) was tested in the presence of GTPgammaS-loaded Cdc42 (5 muM) or PI(4,5)P2-containing vesicles (100 muM; PI(4,5)P2/PI/PC = 10:45:45).	bind
14104	1	5188	7	NULL	NULL	0	NULL	Arp2/3	NULL		bind	NULL				GST-VCA	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_150_6_1299_s_78	10995436	(D) The ability of HT-WG (2 muM) to inhibit the binding of Arp2/3 (0.1 muM) to GST-VCA (0.2 muM) was tested in the presence of GTPgammaS-loaded Cdc42 (5 muM) or PI(4,5)P2-containing vesicles (100 muM; PI(4,5)P2/PI/PC = 10:45:45).	bind
14105	2	5188	7	NULL	NULL	0	NULL	HT-WG	NULL		inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_150_6_1299_s_78	10995436	(D) The ability of HT-WG (2 muM) to inhibit the binding of Arp2/3 (0.1 muM) to GST-VCA (0.2 muM) was tested in the presence of GTPgammaS-loaded Cdc42 (5 muM) or PI(4,5)P2-containing vesicles (100 muM; PI(4,5)P2/PI/PC = 10:45:45).	bind
14001	1	5189	6	NULL	NULL	NULL	NULL	His6-Ap-uch			bind					proteasome	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cell_89_1_115_s_174	9094720	(D) The binding of His6-Ap-uch to the proteasome  reaches saturation.	bind
14106	1	5189	7	NULL	NULL	0	NULL	His6-Ap-uch 	NULL		bind	NULL				proteasome	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_89_1_115_s_174	9094720	(D) The binding of His6-Ap-uch to the proteasome  reaches saturation.	bind
14002	1	5190	6	NULL	NULL	NULL	NULL	p27	GP		bind					cyclin A-cdk2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_13_6058_s_208	15199159	(D) The binding of p27 to cyclin A-cdk2  and skp2 is compromised by the ck( - ) mutation.	bind
14003	2	5190	6	NULL	NULL	NULL	NULL	p27	GP		bind					skp2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_13_6058_s_208	15199159	(D) The binding of p27 to cyclin A-cdk2  and skp2 is compromised by the ck( - ) mutation.	bind
14004	3	5190	6	NULL	NULL	NULL	NULL	statement 1	Process		is compromised by					ck	GP	mutation of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_13_6058_s_208	15199159	(D) The binding of p27 to cyclin A-cdk2  and skp2 is compromised by the ck( - ) mutation.	bind
14005	4	5190	6	NULL	NULL	NULL	NULL	statement 2	Process		is compromised by					ck	GP	mutation of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_13_6058_s_208	15199159	(D) The binding of p27 to cyclin A-cdk2  and skp2 is compromised by the ck( - ) mutation.	bind
14107	1	5190	7	NULL	NULL	0	NULL	p27	NULL		bind	NULL				cyclin A-cdk2	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_13_6058_s_208	15199159	(D) The binding of p27 to cyclin A-cdk2  and skp2 is compromised by the ck( - ) mutation.	bind
14108	2	5190	7	NULL	NULL	0	NULL	p27	NULL		bind	NULL				 skp2 	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_13_6058_s_208	15199159	(D) The binding of p27 to cyclin A-cdk2  and skp2 is compromised by the ck( - ) mutation.	bind
14109	3	5190	7	10	NULL	0	NULL	statement 1	NULL		is compromised by	NULL				ck	NULL	mutation of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_13_6058_s_208	15199159	(D) The binding of p27 to cyclin A-cdk2  and skp2 is compromised by the ck( - ) mutation.	bind
14110	4	5190	7	10	NULL	0	NULL	statement 2	NULL		is compromised by	NULL				ck	NULL	mutation of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_13_6058_s_208	15199159	(D) The binding of p27 to cyclin A-cdk2  and skp2 is compromised by the ck( - ) mutation.	bind
14006	1	5191	6	NULL	NULL	NULL	NULL	ss-affixin	GP	T7-tagged	bind					ILK	GP	FLAG tagged;;point mutants			NULL	COS-7 cells	NULL	NULL	NULL	NULL	gw60_cellbiol_153_6_1251_s_147	11402068	(D) The binding of T7-tagged ss-affixin with Flag-tagged ILK point mutants was examined by immunoprecipitation assays in COS-7 cells.	bind
14111	1	5191	7	10	NULL	0	NULL	ss-affixin	NULL	T7-tagged 	bind	NULL				ILK	NULL	Flag-tagged;;point mutant			NULL	COS-7 cells	NULL	NULL	NULL	NULL	gw60_cellbiol_153_6_1251_s_147	11402068	(D) The binding of T7-tagged ss-affixin with Flag-tagged ILK point mutants was examined by immunoprecipitation assays in COS-7 cells.	bind
14007	1	5192	6	NULL	NULL	NULL	NULL	Comm 	GP	variants	coimmunoprecipates with					Robo	GP				NULL	S2 cells	NULL	NULL	NULL	NULL	gw60_neuron_35_3_447_s_162	12165468	(D) The Comm variants that cannot bind DNedd4 or are not ubiquitinated still coimmunoprecipitate with Robo in S2 cells.	bind
14008	2	5192	6	NULL	NULL	NULL	NULL	Comm 	GP	variants	does not bind					DNedd4	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_35_3_447_s_162	12165468	(D) The Comm variants that cannot bind DNedd4 or are not ubiquitinated still coimmunoprecipitate with Robo in S2 cells.	bind
14009	3	5192	6	NULL	NULL	NULL	NULL	Comm 	GP	variants	is not					ubiquitinated					NULL		NULL	NULL	NULL	NULL	gw60_neuron_35_3_447_s_162	12165468	(D) The Comm variants that cannot bind DNedd4 or are not ubiquitinated still coimmunoprecipitate with Robo in S2 cells.	bind
14112	1	5192	7	NULL	NULL	0	NULL	Comm 	NULL	variants of	does not bind	NULL				DNedd4	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuron_35_3_447_s_162	12165468	(D) The Comm variants that cannot bind DNedd4 or are not ubiquitinated still coimmunoprecipitate with Robo in S2 cells.	bind
14113	2	5192	7	NULL	NULL	0	NULL	Comm 	NULL	variants of	is not	NULL				ubiquitinated	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuron_35_3_447_s_162	12165468	(D) The Comm variants that cannot bind DNedd4 or are not ubiquitinated still coimmunoprecipitate with Robo in S2 cells.	bind
14121	3	5192	7	10	NULL	0	NULL	 Comm	NULL	variants of	coimmunoprecipitate with	NULL				Robo	NULL				NULL	S2 cells	NULL	NULL	NULL	NULL	gw60_neuron_35_3_447_s_162	12165468	(D) The Comm variants that cannot bind DNedd4 or are not ubiquitinated still coimmunoprecipitate with Robo in S2 cells.	bind
14010	1	5193	6	NULL	NULL	NULL	NULL	Daxx	GP		bind			COOH terminus		p53	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_1_322_s_126	12482984	(D) The COOH terminus of Daxx binds to p53.	bind
14120	1	5193	7	NULL	NULL	0	NULL	Daxx	NULL		binds	NULL		COOH terminus		p53	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_1_322_s_126	12482984	(D) The COOH terminus of Daxx binds to p53.	bind
14011	1	5194	6	NULL	NULL	NULL	NULL	depolarization	Process		occurs in response to					cAMP pulse					NULL		NULL	NULL	NULL	NULL	gw60_neuron_36_3_451_s_186	12408847	(D) The depolarization (bottom, solid black trace) in response to a 250 nM cAMP pulse (upper, solid black trace) is due to an accumulation of channels in the open, cAMP-bound state (AO, solid red lines).	bind
14012	2	5194	6	NULL	NULL	NULL	NULL	channels	CellComponent		accumulate in					cAMP-bound state	Process	open			NULL		NULL	NULL	NULL	NULL	gw60_neuron_36_3_451_s_186	12408847	(D) The depolarization (bottom, solid black trace) in response to a 250 nM cAMP pulse (upper, solid black trace) is due to an accumulation of channels in the open, cAMP-bound state (AO, solid red lines).	bind
14013	3	5194	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs due to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_36_3_451_s_186	12408847	(D) The depolarization (bottom, solid black trace) in response to a 250 nM cAMP pulse (upper, solid black trace) is due to an accumulation of channels in the open, cAMP-bound state (AO, solid red lines).	bind
15473	1	5194	7	NULL	NULL	0	NULL	Depolarization	NULL		in response to	NULL				cAMP pulse	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuron_36_3_451_s_186	12408847	(D) The depolarization (bottom, solid black trace) in response to a 250 nM cAMP pulse (upper, solid black trace) is due to an accumulation of channels in the open, cAMP-bound state (AO, solid red lines).	bind
15474	2	5194	7	NULL	NULL	0	NULL	channels	NULL		accumulate in	NULL				 cAMP-bound state 	NULL	open			NULL		NULL	NULL	NULL	NULL	gw60_neuron_36_3_451_s_186	12408847	(D) The depolarization (bottom, solid black trace) in response to a 250 nM cAMP pulse (upper, solid black trace) is due to an accumulation of channels in the open, cAMP-bound state (AO, solid red lines).	bind
19031	3	5194	7	NULL	NULL	0	NULL	statement 1	NULL		due to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_36_3_451_s_186	12408847	(D) The depolarization (bottom, solid black trace) in response to a 250 nM cAMP pulse (upper, solid black trace) is due to an accumulation of channels in the open, cAMP-bound state (AO, solid red lines).	bind
14014	1	5195	6	NULL	NULL	NULL	NULL				does not bind		cooperatively	E7R		TBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_2_397_s_200	12191484	(D) The E7R, E22R POU domain does not cooperatively bind with TBP.	bind
14015	2	5195	6	NULL	NULL	NULL	NULL				does not bind		cooperatively	E22R POU domain		TBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_2_397_s_200	12191484	(D) The E7R, E22R POU domain does not cooperatively bind with TBP.	bind
14122	1	5195	7	10	NULL	0	NULL		NULL		does not bind	NULL	cooperatively	 E7R		TBP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_2_397_s_200	12191484	(D) The E7R, E22R POU domain does not cooperatively bind with TBP.	bind
14123	2	5195	7	10	NULL	0	NULL		NULL		does not bind	NULL	cooperatively	E22R POU domain		TBP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_2_397_s_200	12191484	(D) The E7R, E22R POU domain does not cooperatively bind with TBP.	bind
14016	1	5196	6	NULL	NULL	NULL	NULL	tetrameric IP3 receptor 	GP		bind			four subunits		IP3	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_7_510_s_52	9210378	(d) The Hill coefficients derived from the curves shown in (c) suggest that three and possibly all four subunits of the tetrameric IP3 receptor must bind IP3 before the channel can open and release Ca2+ into the cytosol.	bind
14017	2	5196	6	NULL	NULL	NULL	NULL	channel	CellComponent	open	release					Ca+2 	Chemical				NULL	cytosol	NULL	NULL	NULL	NULL	gw60_currbiol_7_7_510_s_52	9210378	(d) The Hill coefficients derived from the curves shown in (c) suggest that three and possibly all four subunits of the tetrameric IP3 receptor must bind IP3 before the channel can open and release Ca2+ into the cytosol.	bind
14018	3	5196	6	NULL	NULL	NULL	NULL	statement 1	Process		occur before		must			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_7_510_s_52	9210378	(d) The Hill coefficients derived from the curves shown in (c) suggest that three and possibly all four subunits of the tetrameric IP3 receptor must bind IP3 before the channel can open and release Ca2+ into the cytosol.	bind
14124	1	5196	7	10	NULL	0	NULL	tetrameric IP3 receptor	NULL		bind	NULL		four subunits		IP3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_7_510_s_52	9210378	(d) The Hill coefficients derived from the curves shown in (c) suggest that three and possibly all four subunits of the tetrameric IP3 receptor must bind IP3 before the channel can open and release Ca2+ into the cytosol.	bind
14125	2	5196	7	NULL	NULL	0	NULL	channel	NULL	open	release	NULL				Ca2+	NULL				NULL	cytosol	NULL	NULL	NULL	NULL	gw60_currbiol_7_7_510_s_52	9210378	(d) The Hill coefficients derived from the curves shown in (c) suggest that three and possibly all four subunits of the tetrameric IP3 receptor must bind IP3 before the channel can open and release Ca2+ into the cytosol.	bind
14126	3	5196	7	10	NULL	0	NULL	statement 1	NULL		occur before	NULL	must 			statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_7_510_s_52	9210378	(d) The Hill coefficients derived from the curves shown in (c) suggest that three and possibly all four subunits of the tetrameric IP3 receptor must bind IP3 before the channel can open and release Ca2+ into the cytosol.	bind
14019	1	5197	6	NULL	NULL	NULL	NULL	Egr protein	GP		bind					nuclear proteins	GP	mouse;; hippocampus			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10286_s_213	16287845	(D) The mutation within E2m1 completely abrogated Egr protein  binding with nuclear proteins obtained from seized mouse hippocampus.	bind
14020	2	5197	6	NULL	NULL	NULL	NULL	E2m1	GP	mutant	abrogates		completely			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10286_s_213	16287845	(D) The mutation within E2m1 completely abrogated Egr protein  binding with nuclear proteins obtained from seized mouse hippocampus.	bind
14128	1	5197	7	10	NULL	0	NULL	Egr protein 	NULL		bind	NULL				nuclear proteins	NULL	mouse;;hippocampus			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10286_s_213	16287845	(D) The mutation within E2m1 completely abrogated Egr protein  binding with nuclear proteins obtained from seized mouse hippocampus.	bind
14129	2	5197	7	10	NULL	0	NULL	E2m1	NULL	mutant	abrogates	NULL	completely			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10286_s_213	16287845	(D) The mutation within E2m1 completely abrogated Egr protein  binding with nuclear proteins obtained from seized mouse hippocampus.	bind
14021	1	5198	6	NULL	NULL	NULL	NULL	FRS2 protein	GP		bind			PTB domain		TrkA	GP		NPQ pY sequence		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_3_979_s_246	10629055	(D) The PTB domains of FRS2 proteins bind to the NPQ pY sequence of TrkA.	bind
14130	1	5198	7	NULL	NULL	0	NULL	 FRS2 protein	NULL		bind	NULL		PTB domain		TrkA	NULL		NPQ pY sequence 		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_3_979_s_246	10629055	(D) The PTB domains of FRS2 proteins bind to the NPQ pY sequence of TrkA.	bind
14022	1	5199	6	NULL	NULL	NULL	NULL	B-Raf	GP		bind					GST-Rb	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_140	15485920	(D) The Raf-1 peptide is unable to disrupt the binding of  B-Raf to GST-Rb and GST-MEK1 in vitro.	bind
14023	2	5199	6	NULL	NULL	NULL	NULL	B-Raf	GP		bind					GST-MEK1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_140	15485920	(D) The Raf-1 peptide is unable to disrupt the binding of  B-Raf to GST-Rb and GST-MEK1 in vitro.	bind
14024	3	5199	6	NULL	NULL	NULL	NULL	Raf-1 peptide	GP		does not disrupt					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_140	15485920	(D) The Raf-1 peptide is unable to disrupt the binding of  B-Raf to GST-Rb and GST-MEK1 in vitro.	bind
14025	4	5199	6	NULL	NULL	NULL	NULL	Raf-1 peptide	GP		does not disrupt					statement 2	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_140	15485920	(D) The Raf-1 peptide is unable to disrupt the binding of  B-Raf to GST-Rb and GST-MEK1 in vitro.	bind
14131	1	5199	7	NULL	NULL	0	NULL	B-Raf 	NULL		bind	NULL				GST-Rb	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_140	15485920	(D) The Raf-1 peptide is unable to disrupt the binding of  B-Raf to GST-Rb and GST-MEK1 in vitro.	bind
14132	2	5199	7	NULL	NULL	0	NULL	B-Raf 	NULL		bind	NULL				GST-MEK1	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_140	15485920	(D) The Raf-1 peptide is unable to disrupt the binding of  B-Raf to GST-Rb and GST-MEK1 in vitro.	bind
14133	3	5199	7	10	NULL	0	NULL	Raf-1 peptide	NULL		does not disrupt	NULL				statement 1	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_140	15485920	(D) The Raf-1 peptide is unable to disrupt the binding of  B-Raf to GST-Rb and GST-MEK1 in vitro.	bind
14134	4	5199	7	10	NULL	0	NULL	Raf-1 peptide	NULL		does not disrupt	NULL				statement 2	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_140	15485920	(D) The Raf-1 peptide is unable to disrupt the binding of  B-Raf to GST-Rb and GST-MEK1 in vitro.	bind
14026	1	5200	6	NULL	NULL	NULL	NULL	Rip11	GP		bind			C2 domain		PC/PE liposomes	CellComponent	neutral			NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_6_1437_s_50	11163216	(D) The Rip11 C2 domain binds to neutral PC/PE liposomes in a Mg2+-dependent manner.	bind
14027	2	5200	6	NULL	NULL	NULL	NULL	statement 1	Process		is dependent on					Mg+2	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_6_1437_s_50	11163216	(D) The Rip11 C2 domain binds to neutral PC/PE liposomes in a Mg2+-dependent manner.	bind
14135	1	5200	7	NULL	NULL	0	NULL	Rip 11	NULL		binds	NULL		C2 domain		PC/PE liposomes 	NULL	neutral			NULL		0	NULL	NULL	NULL	gw60_molcell_6_6_1437_s_50	11163216	(D) The Rip11 C2 domain binds to neutral PC/PE liposomes in a Mg2+-dependent manner.	bind
14136	2	5200	7	NULL	NULL	0	NULL	statement 1	NULL		depends on	NULL				Mg2+	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_6_6_1437_s_50	11163216	(D) The Rip11 C2 domain binds to neutral PC/PE liposomes in a Mg2+-dependent manner.	bind
14028	1	5201	6	NULL	NULL	NULL	NULL	Rs-Lys2 transcripts	GP		bind		strongly			Rs-Lys2 probe	NucleicAcid	antisense			NULL		NULL	NULL	NULL	NULL	gw70_insectbiochemmolbiol_32_12_1615_s_197	12429113	(D) The Rs-Lys2 transcripts bound strongly to the antisense  Rs-Lys2 probe.	bind
14137	1	5201	7	NULL	NULL	0	NULL	 Rs-Lys2 transcripts	NULL		bind	NULL	strongly			Rs-Lys2 probe	NULL	antisense			NULL		NULL	NULL	NULL	NULL	gw70_insectbiochemmolbiol_32_12_1615_s_197	12429113	(D) The Rs-Lys2 transcripts bound strongly to the antisense  Rs-Lys2 probe.	bind
14029	1	5203	6	NULL	NULL	NULL	NULL	PAI-2	GP		bind			RSL mutant		Rb	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6520_s_155	12944478	(D) The RSL mutant of PAI-2 retains binding to Rb. Input IVT PAI-2 (lane 3, top panel), a C-D interhelical deletion mutant of PAI-2 (C-D PAI-2) (middle panel), or the RSL mutant of PAI-2 (PAI-2Ala380) was incubated with GST-Rb379-928.	bind
14138	1	5203	7	NULL	NULL	0	NULL	PAI-2	NULL		bind	NULL		RSL mutant 		Rb	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_18_6520_s_155	12944478	(D) The RSL mutant of PAI-2 retains binding to Rb. Input IVT PAI-2 (lane 3, top panel), a C-D interhelical deletion mutant of PAI-2 (C-D PAI-2) (middle panel), or the RSL mutant of PAI-2 (PAI-2Ala380) was incubated with GST-Rb379-928.	bind
14030	1	5204	6	NULL	NULL	NULL	NULL	FAK protein	GP		bind					GEX-p85	GP	full-length			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_20_7015_s_121	12242282	(D) The same total cell lysates were also subjected to GST pull-down (PD) assay by using GST fusion protein with full-length p85 (GEX-p85), and the FAK proteins bound to GEX-p85 were detected by immunoblotting with anti-HA antibody.	bind
14139	1	5204	7	NULL	NULL	0	NULL	FAK protein	NULL		bind	NULL				GEX-p85	NULL	full-length			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_20_7015_s_121	12242282	(D) The same total cell lysates were also subjected to GST pull-down (PD) assay by using GST fusion protein with full-length p85 (GEX-p85), and the FAK proteins bound to GEX-p85 were detected by immunoblotting with anti-HA antibody.	bind
14031	1	5205	6	NULL	NULL	NULL	NULL	SAP90	GP		bind			SH3 domain		H6KA2	GP		proline-rich sequences		NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_4_727_s_118	9808460	(D) The SAP90 SH3 domain binds to both proline-rich sequences present in H6KA2(c-term).	bind
14140	1	5205	7	NULL	NULL	0	NULL	SAP90	NULL		binds	NULL		SH3 domain		 H6KA2	NULL		proline-rich sequence in c-term		NULL		0	NULL	NULL	NULL	gw60_neuron_21_4_727_s_118	9808460	(D) The SAP90 SH3 domain binds to both proline-rich sequences present in H6KA2(c-term).	bind
14032	1	5206	6	NULL	NULL	NULL	NULL	Pax2	GP		bind									sequence A5	NULL		NULL	NULL	NULL	NULL	gw70_development_130_13_2903_s_79	12756174	(D) The specificity of Pax2 and Pax6 binding to sequence A5 (lane 1 and 4, -ab) is  confirmed by the addition of anti-Pax2 antibody (lane 2, +P2-ab) and anti-Pax6 antibody  (lane 5, +P6-ab), which inhibits the formation of the complex.	bind
14033	2	5206	6	NULL	NULL	NULL	NULL	Pax6	GP		bind									sequence A5	NULL		NULL	NULL	NULL	NULL	gw70_development_130_13_2903_s_79	12756174	(D) The specificity of Pax2 and Pax6 binding to sequence A5 (lane 1 and 4, -ab) is  confirmed by the addition of anti-Pax2 antibody (lane 2, +P2-ab) and anti-Pax6 antibody  (lane 5, +P6-ab), which inhibits the formation of the complex.	bind
14141	1	5206	7	NULL	NULL	0	NULL	Pax2	NULL		bind	NULL					NULL			sequence A5	NULL		NULL	NULL	NULL	NULL	gw70_development_130_13_2903_s_79	12756174	(D) The specificity of Pax2 and Pax6 binding to sequence A5 (lane 1 and 4, -ab) is  confirmed by the addition of anti-Pax2 antibody (lane 2, +P2-ab) and anti-Pax6 antibody  (lane 5, +P6-ab), which inhibits the formation of the complex.	bind
14142	2	5206	7	NULL	NULL	0	NULL	Pax6 	NULL		bind	NULL					NULL			sequence A5	NULL		NULL	NULL	NULL	NULL	gw70_development_130_13_2903_s_79	12756174	(D) The specificity of Pax2 and Pax6 binding to sequence A5 (lane 1 and 4, -ab) is  confirmed by the addition of anti-Pax2 antibody (lane 2, +P2-ab) and anti-Pax6 antibody  (lane 5, +P6-ab), which inhibits the formation of the complex.	bind
14034	1	5209	6	NULL	NULL	NULL	NULL	carcinoma cells	Cell		carries					CD40	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9806_s_303	16260598	(D) TRAF6 and TRAF2 do not coimmunoprecipitate in  CD40L-stimulated carcinoma cells carrying a mutated CD40 that does not directly bind  TRAF2/TRAF3.	bind
14035	2	5209	6	NULL	NULL	NULL	NULL	TRAF2	GP		does not coimmunoprecipitate in					statement 1	Process	CD40L-stimulated			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9806_s_303	16260598	(D) TRAF6 and TRAF2 do not coimmunoprecipitate in  CD40L-stimulated carcinoma cells carrying a mutated CD40 that does not directly bind  TRAF2/TRAF3.	bind
14095	3	5209	6	NULL	NULL	NULL	NULL	TRAF6	GP		does not coimmuprecipitate in					statement 1	Process	CD40L-stimulated			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9806_s_303	16260598	(D) TRAF6 and TRAF2 do not coimmunoprecipitate in  CD40L-stimulated carcinoma cells carrying a mutated CD40 that does not directly bind  TRAF2/TRAF3.	bind
14096	4	5209	6	NULL	NULL	NULL	NULL	CD40	GP	mutant	does not bind		directly			TRAF2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9806_s_303	16260598	(D) TRAF6 and TRAF2 do not coimmunoprecipitate in  CD40L-stimulated carcinoma cells carrying a mutated CD40 that does not directly bind  TRAF2/TRAF3.	bind
14097	5	5209	6	NULL	NULL	NULL	NULL	CD40	GP	mutant	does not bind		directly			TRAF3	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9806_s_303	16260598	(D) TRAF6 and TRAF2 do not coimmunoprecipitate in  CD40L-stimulated carcinoma cells carrying a mutated CD40 that does not directly bind  TRAF2/TRAF3.	bind
14143	1	5209	7	NULL	NULL	0	NULL	CD40	NULL	mutated	does not bind	NULL	directly			TRAF2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9806_s_303	16260598	(D) TRAF6 and TRAF2 do not coimmunoprecipitate in  CD40L-stimulated carcinoma cells carrying a mutated CD40 that does not directly bind  TRAF2/TRAF3.	bind
15583	2	5209	7	NULL	NULL	0	NULL	CD40	NULL	mutated	does not bind	NULL	directly			TRAF3	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_22_9806_s_303	16260598	(D) TRAF6 and TRAF2 do not coimmunoprecipitate in  CD40L-stimulated carcinoma cells carrying a mutated CD40 that does not directly bind  TRAF2/TRAF3.	bind
15584	3	5209	7	10	NULL	0	NULL	 TRAF6 	NULL		does not coimmunoprecipitate in	NULL				carcinoma cells	NULL	CD40L-stimulated 			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9806_s_303	16260598	(D) TRAF6 and TRAF2 do not coimmunoprecipitate in  CD40L-stimulated carcinoma cells carrying a mutated CD40 that does not directly bind  TRAF2/TRAF3.	bind
15585	4	5209	7	10	NULL	0	NULL	TRAF2	NULL		does not coimmunoprecipitate in	NULL				carcinoma cells	NULL	CD40L-stimulated			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9806_s_303	16260598	(D) TRAF6 and TRAF2 do not coimmunoprecipitate in  CD40L-stimulated carcinoma cells carrying a mutated CD40 that does not directly bind  TRAF2/TRAF3.	bind
15586	5	5209	7	10	NULL	0	NULL	carcinoma cells	NULL		carries	NULL				CD40	NULL	mutated			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9806_s_303	16260598	(D) TRAF6 and TRAF2 do not coimmunoprecipitate in  CD40L-stimulated carcinoma cells carrying a mutated CD40 that does not directly bind  TRAF2/TRAF3.	bind
14036	1	5210	6	NULL	NULL	NULL	NULL	Cd3	GP		bind					Nck	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_109_7_901_s_210	12110186	(D) Transduction of antibody APA1/1 interferes with CD3  binding to Nck. Human PBMC were either mock-transduced or transduced with APA1/1 before stimulation with UCHT1.	bind
14037	2	5210	6	NULL	NULL	NULL	NULL	antibody APA1/1	GP		interferes with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_109_7_901_s_210	12110186	(D) Transduction of antibody APA1/1 interferes with CD3  binding to Nck. Human PBMC were either mock-transduced or transduced with APA1/1 before stimulation with UCHT1.	bind
14147	1	5210	7	NULL	NULL	0	NULL	CD3 	NULL		bind	NULL				Nck	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_109_7_901_s_210	12110186	(D) Transduction of antibody APA1/1 interferes with CD3  binding to Nck. Human PBMC were either mock-transduced or transduced with APA1/1 before stimulation with UCHT1.	bind
14148	2	5210	7	NULL	NULL	0	NULL	antibody APA1/1	NULL		interferes with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_109_7_901_s_210	12110186	(D) Transduction of antibody APA1/1 interferes with CD3  binding to Nck. Human PBMC were either mock-transduced or transduced with APA1/1 before stimulation with UCHT1.	bind
14038	1	5212	6	NULL	NULL	0	NULL	TRIKA1 (Ubc13/Uev1A)	NULL		is 	NULL				E2	NULL	specific			NULL		0	NULL	NULL	NULL	gw60_cell_103_2_351_s_139	11057907	(D) TRIKA1 (Ubc13/Uev1A) is a specific E2 that activates IKK in conjunction with TRAF6.	bind
14039	2	5212	6	NULL	NULL	NULL	NULL	statement 1	Process		activates					IKK	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_2_351_s_139	11057907	(D) TRIKA1 (Ubc13/Uev1A) is a specific E2 that activates IKK in conjunction with TRAF6.	bind
14040	3	5212	6	NULL	NULL	NULL	NULL	TRAF6	GP		activates					IKK	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_2_351_s_139	11057907	(D) TRIKA1 (Ubc13/Uev1A) is a specific E2 that activates IKK in conjunction with TRAF6.	bind
19014	4	5212	6	NULL	NULL	NULL	NULL	statement 2	Process		occurs in conjunction with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_2_351_s_139	11057907	(D) TRIKA1 (Ubc13/Uev1A) is a specific E2 that activates IKK in conjunction with TRAF6.	bind
14151	1	5212	7	NULL	NULL	0	NULL	TRIKA1(Ubc13/Uev1A) 	NULL		activates	NULL				IKK 	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_2_351_s_139	11057907	(D) TRIKA1 (Ubc13/Uev1A) is a specific E2 that activates IKK in conjunction with TRAF6.	bind
14152	2	5212	7	NULL	NULL	0	NULL	TRAF6	NULL		activates	NULL				IKK	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_103_2_351_s_139	11057907	(D) TRIKA1 (Ubc13/Uev1A) is a specific E2 that activates IKK in conjunction with TRAF6.	bind
14153	3	5212	7	NULL	NULL	0	NULL	statement 1	NULL		occurs in conjunction with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_103_2_351_s_139	11057907	(D) TRIKA1 (Ubc13/Uev1A) is a specific E2 that activates IKK in conjunction with TRAF6.	bind
14154	4	5212	7	10	NULL	0	NULL	TRIKA1(Ubc13/Uev1A)	NULL		is	NULL				E2	NULL	specific			NULL		NULL	NULL	NULL	NULL	gw60_cell_103_2_351_s_139	11057907	(D) TRIKA1 (Ubc13/Uev1A) is a specific E2 that activates IKK in conjunction with TRAF6.	bind
14041	1	5213	6	NULL	NULL	NULL	NULL	TrkA	GP		bind		specifically			Kalirin	GP		N-terminal PH domain		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_5106_s_283	15923627	(D) TrkA binds specifically to the N-terminal  PH domains of Kalirin and Trio.	bind
14042	2	5213	6	NULL	NULL	NULL	NULL	TrkA	GP		bind		specifically			Trio	GP		N-terminal PH domain		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_5106_s_283	15923627	(D) TrkA binds specifically to the N-terminal  PH domains of Kalirin and Trio.	bind
14155	1	5213	7	NULL	NULL	0	NULL	TrkA	NULL		binds	NULL	specifically			Kalirin	NULL		N-terminal PH domain		NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_12_5106_s_283	15923627	(D) TrkA binds specifically to the N-terminal  PH domains of Kalirin and Trio.	bind
14156	2	5213	7	NULL	NULL	0	NULL	TrkA	NULL		bind	NULL	specifically			Trio	NULL		N-terminal PH domain		NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_12_5106_s_283	15923627	(D) TrkA binds specifically to the N-terminal  PH domains of Kalirin and Trio.	bind
14043	1	5214	6	NULL	NULL	NULL	NULL	SUV39H1	GP		bind					HP1alpha	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_7_2525_s_355	15767660	(D) TSA did not affect the in vivo binding  of SUV39H1 to HP1alpha as determined by coimmunoprecipitation.	bind
14044	2	5214	6	NULL	NULL	NULL	NULL	TSA	Chemical		did not affect					statement 1	Process				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_7_2525_s_355	15767660	(D) TSA did not affect the in vivo binding  of SUV39H1 to HP1alpha as determined by coimmunoprecipitation.	bind
14157	1	5214	7	NULL	NULL	0	NULL	SUV39H1	NULL		bind	NULL				HP1alpha	NULL				NULL	in vivo	0	NULL	NULL	NULL	gw70_molcellbiol_25_7_2525_s_355	15767660	(D) TSA did not affect the in vivo binding  of SUV39H1 to HP1alpha as determined by coimmunoprecipitation.	bind
14158	2	5214	7	10	NULL	0	NULL	TSA	NULL		does not affect	NULL				statement 1	NULL				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_7_2525_s_355	15767660	(D) TSA did not affect the in vivo binding  of SUV39H1 to HP1alpha as determined by coimmunoprecipitation.	bind
14045	1	5215	6	NULL	NULL	NULL	NULL	VCP	GP		bind					(Ub)2-7 chains					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6469_s_388	12944474	(D) VCP binds to (Ub)2-7 chains more weakly than ataxin-3.	bind
14046	2	5215	6	NULL	NULL	NULL	NULL	ataxin-3	GP		bind					(Ub)2-7 chains					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6469_s_388	12944474	(D) VCP binds to (Ub)2-7 chains more weakly than ataxin-3.	bind
14047	3	5215	6	NULL	NULL	NULL	NULL	statement 1	Process		is weaker than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6469_s_388	12944474	(D) VCP binds to (Ub)2-7 chains more weakly than ataxin-3.	bind
14159	1	5215	7	10	NULL	0	NULL	VCP	NULL		binds	NULL				(Ub)2-7 chains	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6469_s_388	12944474	(D) VCP binds to (Ub)2-7 chains more weakly than ataxin-3.	bind
14160	2	5215	7	10	NULL	0	NULL	ataxin-3	NULL		binds	NULL				(Ub)2-7 chains	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6469_s_388	12944474	(D) VCP binds to (Ub)2-7 chains more weakly than ataxin-3.	bind
14161	3	5215	7	NULL	NULL	0	NULL	statement 1	NULL		occurs	NULL				statement 2	NULL	more weakly than			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6469_s_388	12944474	(D) VCP binds to (Ub)2-7 chains more weakly than ataxin-3.	bind
14048	1	5216	6	NULL	NULL	NULL	NULL	VP16	GP		bind					HCF-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_14_4700_s_279	11416146	(D) VP16 binding to HCF-1 was assayed as described in the legend to Fig.  6.	bind
14162	1	5216	7	NULL	NULL	0	NULL	VP16	NULL		bind	NULL				HCF-1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_14_4700_s_279	11416146	(D) VP16 binding to HCF-1 was assayed as described in the legend to Fig.  6.	bind
14049	1	5217	6	NULL	NULL	NULL	NULL	Vsm1	GP		bind					Sso1	GP	native			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_8_3114_s_202	12925750	(D) Vsm1 binds better to native Sso1 than constitutively open mutants.	bind
19015	2	5217	6	NULL	NULL	NULL	NULL	Vsm1	GP		bind					Sso1	GP	constitutively open mutant			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_8_3114_s_202	12925750	(D) Vsm1 binds better to native Sso1 than constitutively open mutants.	bind
19016	3	5217	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs better than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_8_3114_s_202	12925750	(D) Vsm1 binds better to native Sso1 than constitutively open mutants.	bind
14163	1	5217	7	NULL	NULL	0	NULL	Vsm1	NULL		binds	NULL				Sso1	NULL	native			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_8_3114_s_202	12925750	(D) Vsm1 binds better to native Sso1 than constitutively open mutants.	bind
14164	2	5217	7	NULL	NULL	0	NULL	Vsm1	NULL		binds	NULL				Sso1	NULL	constitutively open mutant			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_8_3114_s_202	12925750	(D) Vsm1 binds better to native Sso1 than constitutively open mutants.	bind
14165	3	5217	7	NULL	NULL	0	NULL	statement 1	NULL		occurs better than 	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_8_3114_s_202	12925750	(D) Vsm1 binds better to native Sso1 than constitutively open mutants.	bind
14114	1	5220	6	NULL	NULL	NULL	NULL	GCP2	GP		bind					pericentrin A fragment	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_8_3642_s_121	15146056	(D) Yeast two-hybrid data showing binding of GCP2  by a pericentrin A fragment and lack of GCP2 binding by the homologous pericentrin  B fragment as well as mutants lacking a pericentrin B specific exon (see MATERIALS  AND METHODS for details).	bind
14115	2	5220	6	NULL	NULL	NULL	NULL	pericentrin B fragment	GP	homologous	does not bind					GCP2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_8_3642_s_121	15146056	(D) Yeast two-hybrid data showing binding of GCP2  by a pericentrin A fragment and lack of GCP2 binding by the homologous pericentrin  B fragment as well as mutants lacking a pericentrin B specific exon (see MATERIALS  AND METHODS for details).	bind
14116	3	5220	6	NULL	NULL	NULL	NULL	eletion	GP	mutant	does not bind				pericentrin B specific exon	GCP2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_8_3642_s_121	15146056	(D) Yeast two-hybrid data showing binding of GCP2  by a pericentrin A fragment and lack of GCP2 binding by the homologous pericentrin  B fragment as well as mutants lacking a pericentrin B specific exon (see MATERIALS  AND METHODS for details).	bind
14168	1	5220	7	NULL	NULL	0	NULL	GCP2	NULL		bind	NULL				pericentrin A fragment 	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_8_3642_s_121	15146056	(D) Yeast two-hybrid data showing binding of GCP2  by a pericentrin A fragment and lack of GCP2 binding by the homologous pericentrin  B fragment as well as mutants lacking a pericentrin B specific exon (see MATERIALS  AND METHODS for details).	bind
14169	2	5220	7	NULL	NULL	0	NULL	GCP2	NULL		does not bind	NULL				pericentrin B fragment	NULL	homologous			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_8_3642_s_121	15146056	(D) Yeast two-hybrid data showing binding of GCP2  by a pericentrin A fragment and lack of GCP2 binding by the homologous pericentrin  B fragment as well as mutants lacking a pericentrin B specific exon (see MATERIALS  AND METHODS for details).	bind
14170	3	5220	7	NULL	NULL	0	NULL	GCP2	NULL		does not bind	NULL					NULL	mutant		pericentrin B specific exon	NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_8_3642_s_121	15146056	(D) Yeast two-hybrid data showing binding of GCP2  by a pericentrin A fragment and lack of GCP2 binding by the homologous pericentrin  B fragment as well as mutants lacking a pericentrin B specific exon (see MATERIALS  AND METHODS for details).	bind
14117	1	5221	6	NULL	NULL	NULL	NULL	Smad4	GP	nuclear	bind					DNA	NucleicAcid			SBE	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_13_4494_s_182	12808092	(D) YY1  inhibits binding of nuclear Smad4 to SBE DNA.	bind
14118	2	5221	6	NULL	NULL	NULL	NULL	YY1	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_13_4494_s_182	12808092	(D) YY1  inhibits binding of nuclear Smad4 to SBE DNA.	bind
14171	1	5221	7	NULL	NULL	0	NULL	Smad4	NULL	nuclear	binds	NULL				DNA	NULL			SBE	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_13_4494_s_182	12808092	(D) YY1  inhibits binding of nuclear Smad4 to SBE DNA.	bind
14172	2	5221	7	NULL	NULL	0	NULL	YY1	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_13_4494_s_182	12808092	(D) YY1  inhibits binding of nuclear Smad4 to SBE DNA.	bind
14119	1	5225	6	NULL	NULL	NULL	NULL	sgt1-3 protein	GP		does not bind					Hsc82	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_18_8069_s_233	15340069	(D, top) sgt1-3 protein (sgt1-3p) does  not bind to Hsc82 in vitro.	bind
19017	2	5225	6	NULL	NULL	NULL	NULL	sgt1-3p	GP		is					sgt1-3 protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_18_8069_s_233	15340069	(D, top) sgt1-3 protein (sgt1-3p) does  not bind to Hsc82 in vitro.	bind
14173	1	5225	7	NULL	NULL	0	NULL	sgt1-3p	NULL		does not bind	NULL				Hsc82	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw70_molcellbiol_24_18_8069_s_233	15340069	(D, top) sgt1-3 protein (sgt1-3p) does  not bind to Hsc82 in vitro.	bind
14174	2	5225	7	NULL	NULL	0	NULL	sgt1-3p	NULL		is	NULL				sgt1-3 protein	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_18_8069_s_233	15340069	(D, top) sgt1-3 protein (sgt1-3p) does  not bind to Hsc82 in vitro.	bind
14812	1	5226	6	NULL	NULL	NULL	NULL	Pcl2	GP	chick	downregulates					Shh	GP				NULL	embryos	NULL	NULL	NULL	NULL	gw70_development_131_17_4381_s_188	15294861	(D,F,H,J) Embryos overexpressing chick  Pcl2 show downregulation of  Shh (D) in the node and notochord, of  Nodal (F) and  Pitx2 (H) in the left LPM, and of  Lefty1 (J) in the prospective floor plate.	bind
15475	1	5226	7	NULL	NULL	0	NULL	Pcl2	NULL	chick	downregulates	NULL				Shh	NULL				NULL	embryos	NULL	NULL	NULL	NULL	gw70_development_131_17_4381_s_188	15294861	(D,F,H,J) Embryos overexpressing chick  Pcl2 show downregulation of  Shh (D) in the node and notochord, of  Nodal (F) and  Pitx2 (H) in the left LPM, and of  Lefty1 (J) in the prospective floor plate.	bind
14183	1	5227	6	NULL	NULL	NULL	NULL	ORC	GP		bind		significantly			ars1 DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_24_13589_s_110	11717425	(dI-dC) also reduced ORC binding to  ars1 DNA significantly (plateauing at  90% inhibition at high levels).	bind
14175	1	5227	7	10	NULL	0	NULL	ORC	NULL		bind	NULL	significantly			 ars1 DNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_24_13589_s_110	11717425	(dI-dC) also reduced ORC binding to  ars1 DNA significantly (plateauing at  90% inhibition at high levels).	bind
14184	1	5228	6	NULL	NULL	NULL	NULL	VAB-1-AP	GP		bind		specifically			VAB-2/EFN-1 expressing cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_cell_99_7_781_s_84	10619431	(E - G) VAB-1-AP specifically binds to VAB-2/EFN-1 expressing cells.	bind
14176	1	5228	7	NULL	NULL	0	NULL	VAB-1-AP	NULL		binds	NULL	specifically			VAB-2/EFN-1 expressing cells	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_99_7_781_s_84	10619431	(E - G) VAB-1-AP specifically binds to VAB-2/EFN-1 expressing cells.	bind
14185	1	5230	6	NULL	NULL	NULL	NULL	E.coli	Organism		bind					BEC	Cell	human			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_4_1947_s_143	15784534	(E and F) Binding of  E. coli to human BECs visualized by staining with crystal violet.	bind
14177	1	5230	7	NULL	NULL	0	NULL	E. coli 	NULL		binds	NULL				BECs	NULL	human			NULL		0	NULL	NULL	NULL	gw70_infectimmun_73_4_1947_s_143	15784534	(E and F) Binding of  E. coli to human BECs visualized by staining with crystal violet.	bind
14186	1	5231	6	NULL	NULL	NULL	NULL	C/EBP-alpha	GP		bind					NP-3	GP			promoter sequences	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_322_s_104	9418879	(E and F) Binding of C/EBP-alpha to NP-3 promoter sequences.	bind
14178	1	5231	7	NULL	NULL	0	NULL	C/EBP-alpha	NULL		binds	NULL				NP-3 	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_322_s_104	9418879	(E and F) Binding of C/EBP-alpha to NP-3 promoter sequences.	bind
14813	1	5232	6	NULL	NULL	NULL	NULL	DNase I	GP	purified;;fluorescein labeled	bind					G-actin	GP	unlabeled chicken			NULL		NULL	NULL	NULL	NULL	gw70_devbiol_271_1_59_s_377	15196950	(E and F) Control zygote microinjected  with rhodamine-labeled G-actin at stage 0.1 and with purified fluorescein-labeled  DNase I bound to unlabeled chicken G-actin at stage 0.8.	bind
19018	2	5232	6	NULL	NULL	NULL	NULL	G-actin	GP	rhodamine-labeled	bind					G-actin	GP	unlabeled chicken			NULL		NULL	NULL	NULL	NULL	gw70_devbiol_271_1_59_s_377	15196950	(E and F) Control zygote microinjected  with rhodamine-labeled G-actin at stage 0.1 and with purified fluorescein-labeled  DNase I bound to unlabeled chicken G-actin at stage 0.8.	bind
14179	1	5232	7	NULL	NULL	0	NULL	G-actin 	NULL	rhodamine-labeled	bind	NULL				G-actin	NULL	unlabeled chicken			NULL		0	NULL	NULL	NULL	gw70_devbiol_271_1_59_s_377	15196950	(E and F) Control zygote microinjected  with rhodamine-labeled G-actin at stage 0.1 and with purified fluorescein-labeled  DNase I bound to unlabeled chicken G-actin at stage 0.8.	bind
14180	2	5232	7	10	NULL	0	NULL	DNase I	NULL	purified;;fluorescein-labeled	bind	NULL				G-actin	NULL	unlabeled chicken 			NULL		NULL	NULL	NULL	NULL	gw70_devbiol_271_1_59_s_377	15196950	(E and F) Control zygote microinjected  with rhodamine-labeled G-actin at stage 0.1 and with purified fluorescein-labeled  DNase I bound to unlabeled chicken G-actin at stage 0.8.	bind
14187	1	5234	6	NULL	NULL	NULL	NULL	His-GFP-SsrA protein	GP		bind					SspB	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_75_s_51	12887894	(E and F) Isothermal titration calorimetric studies of His-GFP-SsrA protein binding to SspB (E) and SspB127 (F) reveal dissociation constants of 728 and 695 nM, respectively.	bind
14188	2	5234	6	NULL	NULL	NULL	NULL	His-GFP-SsrA protein	GP		bind					SspB127	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_75_s_51	12887894	(E and F) Isothermal titration calorimetric studies of His-GFP-SsrA protein binding to SspB (E) and SspB127 (F) reveal dissociation constants of 728 and 695 nM, respectively.	bind
14181	1	5234	7	NULL	NULL	0	NULL	His-GFP-SsrA	NULL		bind	NULL				SspB	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_12_1_75_s_51	12887894	(E and F) Isothermal titration calorimetric studies of His-GFP-SsrA protein binding to SspB (E) and SspB127 (F) reveal dissociation constants of 728 and 695 nM, respectively.	bind
14182	2	5234	7	NULL	NULL	0	NULL	His-GFP-SsrA	NULL		bind	NULL				SspB127	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_12_1_75_s_51	12887894	(E and F) Isothermal titration calorimetric studies of His-GFP-SsrA protein binding to SspB (E) and SspB127 (F) reveal dissociation constants of 728 and 695 nM, respectively.	bind
14814	1	5236	6	NULL	NULL	NULL	NULL	IFNAR1-EC	GP		bind					IFNAR1-EC receptor surface	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_5_1888_s_28	16479007	(E to G) Dissociation  of wt IFN-alpha2 (E), IFN-beta (F), and the HEQ mutant (G) from the ternary complex, with both IFNAR1-EC  and IFNAR2-EC bound to the surface (IFNAR2-EC I47A was used for IFN-beta), at IFNAR1-EC  receptor surface concentrations of 4 fmol/mm2 (black), 2 fmol/mm2 (red), and 1 fmol/mm2 (blue).	bind
14815	2	5236	6	NULL	NULL	NULL	NULL	IFNAR2-EC	GP		bind					IFNAR1-EC receptor surface	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_5_1888_s_28	16479007	(E to G) Dissociation  of wt IFN-alpha2 (E), IFN-beta (F), and the HEQ mutant (G) from the ternary complex, with both IFNAR1-EC  and IFNAR2-EC bound to the surface (IFNAR2-EC I47A was used for IFN-beta), at IFNAR1-EC  receptor surface concentrations of 4 fmol/mm2 (black), 2 fmol/mm2 (red), and 1 fmol/mm2 (blue).	bind
16181	3	5236	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs simultaneously with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_5_1888_s_28	16479007	(E to G) Dissociation  of wt IFN-alpha2 (E), IFN-beta (F), and the HEQ mutant (G) from the ternary complex, with both IFNAR1-EC  and IFNAR2-EC bound to the surface (IFNAR2-EC I47A was used for IFN-beta), at IFNAR1-EC  receptor surface concentrations of 4 fmol/mm2 (black), 2 fmol/mm2 (red), and 1 fmol/mm2 (blue).	bind
16182	4	5236	6	NULL	NULL	NULL	NULL	IFN-alpha2	GP	wt	dissociates from					ternary complex					NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_5_1888_s_28	16479007	(E to G) Dissociation  of wt IFN-alpha2 (E), IFN-beta (F), and the HEQ mutant (G) from the ternary complex, with both IFNAR1-EC  and IFNAR2-EC bound to the surface (IFNAR2-EC I47A was used for IFN-beta), at IFNAR1-EC  receptor surface concentrations of 4 fmol/mm2 (black), 2 fmol/mm2 (red), and 1 fmol/mm2 (blue).	bind
16183	5	5236	6	NULL	NULL	NULL	NULL	IFN-beta	GP		dissociates from					ternary complex					NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_5_1888_s_28	16479007	(E to G) Dissociation  of wt IFN-alpha2 (E), IFN-beta (F), and the HEQ mutant (G) from the ternary complex, with both IFNAR1-EC  and IFNAR2-EC bound to the surface (IFNAR2-EC I47A was used for IFN-beta), at IFNAR1-EC  receptor surface concentrations of 4 fmol/mm2 (black), 2 fmol/mm2 (red), and 1 fmol/mm2 (blue).	bind
16184	6	5236	6	10	NULL	0	NULL		NULL	mutant	dissociates from	NULL		HEQ		ternary complex	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_5_1888_s_28	16479007	(E to G) Dissociation  of wt IFN-alpha2 (E), IFN-beta (F), and the HEQ mutant (G) from the ternary complex, with both IFNAR1-EC  and IFNAR2-EC bound to the surface (IFNAR2-EC I47A was used for IFN-beta), at IFNAR1-EC  receptor surface concentrations of 4 fmol/mm2 (black), 2 fmol/mm2 (red), and 1 fmol/mm2 (blue).	bind
15108	1	5236	7	NULL	NULL	0	NULL	 IFN-alpha2 	NULL	wt	dissociates from	NULL				ternary complex	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_5_1888_s_28	16479007	(E to G) Dissociation  of wt IFN-alpha2 (E), IFN-beta (F), and the HEQ mutant (G) from the ternary complex, with both IFNAR1-EC  and IFNAR2-EC bound to the surface (IFNAR2-EC I47A was used for IFN-beta), at IFNAR1-EC  receptor surface concentrations of 4 fmol/mm2 (black), 2 fmol/mm2 (red), and 1 fmol/mm2 (blue).	bind
15109	2	5236	7	10	NULL	0	NULL	IFN-beta 	NULL		dissociates from	NULL				ternary complex	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_5_1888_s_28	16479007	(E to G) Dissociation  of wt IFN-alpha2 (E), IFN-beta (F), and the HEQ mutant (G) from the ternary complex, with both IFNAR1-EC  and IFNAR2-EC bound to the surface (IFNAR2-EC I47A was used for IFN-beta), at IFNAR1-EC  receptor surface concentrations of 4 fmol/mm2 (black), 2 fmol/mm2 (red), and 1 fmol/mm2 (blue).	bind
15110	3	5236	7	10	NULL	0	NULL		NULL	mutant	dissociates from	NULL		HEQ		ternary complex	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_5_1888_s_28	16479007	(E to G) Dissociation  of wt IFN-alpha2 (E), IFN-beta (F), and the HEQ mutant (G) from the ternary complex, with both IFNAR1-EC  and IFNAR2-EC bound to the surface (IFNAR2-EC I47A was used for IFN-beta), at IFNAR1-EC  receptor surface concentrations of 4 fmol/mm2 (black), 2 fmol/mm2 (red), and 1 fmol/mm2 (blue).	bind
15111	4	5236	7	NULL	NULL	0	NULL	IFNAR1-EC	NULL		bind	NULL				IFNAR1-EC receptor surface	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_5_1888_s_28	16479007	(E to G) Dissociation  of wt IFN-alpha2 (E), IFN-beta (F), and the HEQ mutant (G) from the ternary complex, with both IFNAR1-EC  and IFNAR2-EC bound to the surface (IFNAR2-EC I47A was used for IFN-beta), at IFNAR1-EC  receptor surface concentrations of 4 fmol/mm2 (black), 2 fmol/mm2 (red), and 1 fmol/mm2 (blue).	bind
15112	5	5236	7	NULL	NULL	0	NULL	IFNAR2-EC	NULL		bind	NULL				IFNAR1-EC receptor surface	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_5_1888_s_28	16479007	(E to G) Dissociation  of wt IFN-alpha2 (E), IFN-beta (F), and the HEQ mutant (G) from the ternary complex, with both IFNAR1-EC  and IFNAR2-EC bound to the surface (IFNAR2-EC I47A was used for IFN-beta), at IFNAR1-EC  receptor surface concentrations of 4 fmol/mm2 (black), 2 fmol/mm2 (red), and 1 fmol/mm2 (blue).	bind
15594	6	5236	7	NULL	NULL	0	NULL	statement 4	NULL		occurs simultaneous with	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_5_1888_s_28	16479007	(E to G) Dissociation  of wt IFN-alpha2 (E), IFN-beta (F), and the HEQ mutant (G) from the ternary complex, with both IFNAR1-EC  and IFNAR2-EC bound to the surface (IFNAR2-EC I47A was used for IFN-beta), at IFNAR1-EC  receptor surface concentrations of 4 fmol/mm2 (black), 2 fmol/mm2 (red), and 1 fmol/mm2 (blue).	bind
14341	1	5237	6	NULL	NULL	NULL	NULL	HRX	GP		bind					GADD34	GP	endogenous			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_7050_s_173	10490642	(E to G) HRX fusion proteins bind endogenous GADD34 in vivo.	bind
44686	2	5237	6	NULL	NULL	NULL	NULL	HRX	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_7050_s_173	10490642	(E to G) HRX fusion proteins bind endogenous GADD34 in vivo.	bind
15113	1	5237	7	10	NULL	0	NULL	HRX	NULL		bind	NULL				GADD34	NULL	endogenous			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_10_7050_s_173	10490642	(E to G) HRX fusion proteins bind endogenous GADD34 in vivo.	bind
44687	3	5237	7	10	NULL	0	NULL	HRX	NULL		is a type of	NULL				fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_10_7050_s_173	10490642	(E to G) HRX fusion proteins bind endogenous GADD34 in vivo.	bind
14342	1	5238	6	NULL	NULL	NULL	NULL	35S-A-Raf	GP		does not bind					GST-Rb	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_141	15485920	(E) 35S-A-Raf does not bind to GST-Rb but binds to the positive control GST-MEK1.	bind
14343	2	5238	6	NULL	NULL	NULL	NULL	35S-A-Raf	GP		bind					GST-MEK1	GP	positive control			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_141	15485920	(E) 35S-A-Raf does not bind to GST-Rb but binds to the positive control GST-MEK1.	bind
15114	1	5238	7	NULL	NULL	0	NULL	35S-A-Raf	NULL		does not bind	NULL				GST-Rb	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_141	15485920	(E) 35S-A-Raf does not bind to GST-Rb but binds to the positive control GST-MEK1.	bind
15115	2	5238	7	10	NULL	0	NULL	35S-A-Raf	NULL		bind	NULL				GST-MEK1	NULL	positive control			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_141	15485920	(E) 35S-A-Raf does not bind to GST-Rb but binds to the positive control GST-MEK1.	bind
14344	1	5240	6	NULL	NULL	NULL	NULL	Ad2	GP		bind		specifically			M21-L4 litter cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_158_6_1119_s_98	12221069	(E) Ad2 binds specifically to both M21-L4 and M21 litter cells.	bind
14345	2	5240	6	NULL	NULL	NULL	NULL	Ad2	GP		bind		specifically			M21 litter cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_158_6_1119_s_98	12221069	(E) Ad2 binds specifically to both M21-L4 and M21 litter cells.	bind
15116	1	5240	7	NULL	NULL	0	NULL	Ad2	NULL		binds	NULL	specifically			M21-L4 cells	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_158_6_1119_s_98	12221069	(E) Ad2 binds specifically to both M21-L4 and M21 litter cells.	bind
15117	2	5240	7	NULL	NULL	0	NULL	Ad2	NULL		binds	NULL	specifically			M21 litter cells	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_158_6_1119_s_98	12221069	(E) Ad2 binds specifically to both M21-L4 and M21 litter cells.	bind
14346	1	5241	6	NULL	NULL	NULL	NULL	KLC-1	GP		bind					calsyntenin-1	GP	point mutants			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_8_3651_s_163	16760430	(E) Analysis of KLC1-binding of calsyntenin-1 point mutants by quantitative GST  pulldown assay.	bind
15118	1	5241	7	NULL	NULL	0	NULL	KLC1	NULL		bind	NULL				calsyntenin-1	NULL	point mutant			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_8_3651_s_163	16760430	(E) Analysis of KLC1-binding of calsyntenin-1 point mutants by quantitative GST  pulldown assay.	bind
14347	1	5243	6	NULL	NULL	NULL	NULL	ATF6	GP		bind									ATF6 site	NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_881_s_253	11779464	(E) Binding  of ATF6 and XBP1 to the ATF6  site.	bind
14348	2	5243	6	NULL	NULL	NULL	NULL	XBP1	GP		bind									ATF6 site	NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_881_s_253	11779464	(E) Binding  of ATF6 and XBP1 to the ATF6  site.	bind
15119	1	5243	7	NULL	NULL	0	NULL	ATF6	NULL		bind	NULL					NULL			ATF6 site	NULL		0	NULL	NULL	NULL	gw60_cell_107_7_881_s_253	11779464	(E) Binding  of ATF6 and XBP1 to the ATF6  site.	bind
15120	2	5243	7	NULL	NULL	0	NULL	XBP1	NULL		bind	NULL					NULL			ATF6 site	NULL		0	NULL	NULL	NULL	gw60_cell_107_7_881_s_253	11779464	(E) Binding  of ATF6 and XBP1 to the ATF6  site.	bind
14349	1	5244	6	NULL	NULL	NULL	NULL	E2F1	GP	endogenous;;cellular lysates	bind					GST-Phb	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_312_2_459_s_98	14637159	(E) Binding  of endogenous E2F1 present in cellular lysates to GST-Phb and GST-Phb-CC beads in  vitro; the binding was detected by Western blotting.	bind
14350	2	5244	6	NULL	NULL	NULL	NULL	E2F1	GP	endogenous;;cellular lysates	bind					GST-Phb-CC	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_312_2_459_s_98	14637159	(E) Binding  of endogenous E2F1 present in cellular lysates to GST-Phb and GST-Phb-CC beads in  vitro; the binding was detected by Western blotting.	bind
15121	1	5244	7	10	NULL	0	NULL	E2F1	NULL	endogenous;;cellular lysates	bind	NULL				GST-Phb	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_312_2_459_s_98	14637159	(E) Binding  of endogenous E2F1 present in cellular lysates to GST-Phb and GST-Phb-CC beads in  vitro; the binding was detected by Western blotting.	bind
15122	2	5244	7	10	NULL	0	NULL	E2F1	NULL	endogenous;;cellular lysates	bind	NULL				GST-Phb-CC	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_312_2_459_s_98	14637159	(E) Binding  of endogenous E2F1 present in cellular lysates to GST-Phb and GST-Phb-CC beads in  vitro; the binding was detected by Western blotting.	bind
14351	1	5245	6	NULL	NULL	NULL	NULL	SLP-76	GP		bind					Vav	GP				NULL	jurkat cells	NULL	NULL	NULL	NULL	gw60_immunity_6_2_155_s_190	9047237	(E) Binding between SLP-76 and Vav in Jurkat cells.	bind
15123	1	5245	7	NULL	NULL	0	NULL	SLP-76	NULL		bind	NULL				Vav	NULL				NULL	Jurkat cells	0	NULL	NULL	NULL	gw60_immunity_6_2_155_s_190	9047237	(E) Binding between SLP-76 and Vav in Jurkat cells.	bind
14352	1	5246	6	NULL	NULL	NULL	NULL	Ad4BP/SF-1	GP		bind									XRE site	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_10040_s_288	16260617	(E) Binding of Ad4BP/SF-1 to  the XRE and Ad4 sites in the presence or absence of AhR, revealed by ChIP assays.	bind
14353	2	5246	6	NULL	NULL	NULL	NULL	Ad4BP/SF-1	GP		bind									Ad4 site	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_10040_s_288	16260617	(E) Binding of Ad4BP/SF-1 to  the XRE and Ad4 sites in the presence or absence of AhR, revealed by ChIP assays.	bind
15124	1	5246	7	NULL	NULL	0	NULL	Ad4BP/SF-1	NULL		bind	NULL					NULL			Ad4 site	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_22_10040_s_288	16260617	(E) Binding of Ad4BP/SF-1 to  the XRE and Ad4 sites in the presence or absence of AhR, revealed by ChIP assays.	bind
15125	2	5246	7	NULL	NULL	0	NULL	Ad4BP/SF-1	NULL		bind	NULL					NULL			 XRE site 	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_22_10040_s_288	16260617	(E) Binding of Ad4BP/SF-1 to  the XRE and Ad4 sites in the presence or absence of AhR, revealed by ChIP assays.	bind
14354	1	5247	6	NULL	NULL	NULL	NULL	Adf-1	GP		bind					ftz	GP	proximal		enhancer	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_6_3384_s_242	9584179	(E) Binding of Adf-1 to the  ftz proximal enhancer and that to the Adh distal promoter sites were compared.	bind
14355	2	5247	6	NULL	NULL	NULL	NULL	Adf-1	GP		bind					Adh	GP	distal		promoter 	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_6_3384_s_242	9584179	(E) Binding of Adf-1 to the  ftz proximal enhancer and that to the Adh distal promoter sites were compared.	bind
15126	1	5247	7	10	NULL	0	NULL	Adf-1	NULL		bind	NULL				 ftz	NULL	proximal		enhancer	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_6_3384_s_242	9584179	(E) Binding of Adf-1 to the  ftz proximal enhancer and that to the Adh distal promoter sites were compared.	bind
15127	2	5247	7	10	NULL	0	NULL	Adf-1	NULL		bind	NULL				Adh 	NULL	distal		promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_6_3384_s_242	9584179	(E) Binding of Adf-1 to the  ftz proximal enhancer and that to the Adh distal promoter sites were compared.	bind
14356	1	5248	6	NULL	NULL	NULL	NULL	C3dg-SA-PE	GP		bind					B cells	Cell	splenic			NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_6_713_s_74	12479818	(E) Binding of C3dg-SA-PE to splenic B cells.	bind
15128	1	5248	7	NULL	NULL	0	NULL	C3dg-SA-PE	NULL		bind	NULL				B cells	NULL	splenic			NULL		0	NULL	NULL	NULL	gw60_immunity_17_6_713_s_74	12479818	(E) Binding of C3dg-SA-PE to splenic B cells.	bind
14357	1	5249	6	NULL	NULL	NULL	NULL	Dpr	GP		bind			PDZ-B		XDsh	GP		PDZ		NULL		NULL	NULL	NULL	NULL	gw60_devcell_2_4_449_s_90	11970895	(E) Binding of Dpr PDZ-B to XDsh PDZ.	bind
15129	1	5249	7	NULL	NULL	0	NULL	Dpr 	NULL		bind	NULL		PDZ-B		XDsh	NULL		PDZ		NULL		0	NULL	NULL	NULL	gw60_devcell_2_4_449_s_90	11970895	(E) Binding of Dpr PDZ-B to XDsh PDZ.	bind
14816	1	5250	6	NULL	NULL	NULL	NULL	Mgamma proteins	GP		bind					B1 probe	NucleicAcid	labeled			NULL	soluble bacterial extract	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4600_s_111	10373509	(E) Binding of Mgamma and Mbeta proteins (approximately 50 ng of pGex fusion protein in a soluble bacterial extract) to labeled B1 probe in the presence of nonspecific competitor DNA [poly(dI-dC)] or 5-, 10-, 20-, or 40-fold molar excess of unlabeled B1, N-box, or Hairy oligonucleotide as indicated.	bind
14817	2	5250	6	NULL	NULL	NULL	NULL	Mbeta proteins	GP		bind					B1 probe	NucleicAcid	labeled			NULL	soluble bacterial extract	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4600_s_111	10373509	(E) Binding of Mgamma and Mbeta proteins (approximately 50 ng of pGex fusion protein in a soluble bacterial extract) to labeled B1 probe in the presence of nonspecific competitor DNA [poly(dI-dC)] or 5-, 10-, 20-, or 40-fold molar excess of unlabeled B1, N-box, or Hairy oligonucleotide as indicated.	bind
15130	1	5250	7	10	NULL	0	NULL	Mgamma proteins	NULL		bind	NULL				B1 probe 	NULL	labeled			NULL	soluble bacterial extract	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4600_s_111	10373509	(E) Binding of Mgamma and Mbeta proteins (approximately 50 ng of pGex fusion protein in a soluble bacterial extract) to labeled B1 probe in the presence of nonspecific competitor DNA [poly(dI-dC)] or 5-, 10-, 20-, or 40-fold molar excess of unlabeled B1, N-box, or Hairy oligonucleotide as indicated.	bind
15131	2	5250	7	10	NULL	0	NULL	Mbeta proteins	NULL		bind	NULL				B1 probe 	NULL	labeled			NULL	soluble bacterial extract	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4600_s_111	10373509	(E) Binding of Mgamma and Mbeta proteins (approximately 50 ng of pGex fusion protein in a soluble bacterial extract) to labeled B1 probe in the presence of nonspecific competitor DNA [poly(dI-dC)] or 5-, 10-, 20-, or 40-fold molar excess of unlabeled B1, N-box, or Hairy oligonucleotide as indicated.	bind
14358	1	5251	6	NULL	NULL	NULL	NULL	myosin-Va	GP		bind					syntaxin-1A	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_101	16030255	(E) Binding of myosin-Va by syntaxin-1A requires ATP analogues in presence of 10 - 6 M Ca2+.	bind
14359	2	5251	6	NULL	NULL	NULL	NULL	statement 1	Process		requires					ATP analogues	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_101	16030255	(E) Binding of myosin-Va by syntaxin-1A requires ATP analogues in presence of 10 - 6 M Ca2+.	bind
14360	3	5251	6	NULL	NULL	NULL	NULL	statement 2	Process		occurs in presence of					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_101	16030255	(E) Binding of myosin-Va by syntaxin-1A requires ATP analogues in presence of 10 - 6 M Ca2+.	bind
15132	1	5251	7	NULL	NULL	0	NULL	myosin-Va	NULL		bind	NULL				syntaxin-1A	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_101	16030255	(E) Binding of myosin-Va by syntaxin-1A requires ATP analogues in presence of 10 - 6 M Ca2+.	bind
15133	2	5251	7	NULL	NULL	0	NULL	statement 1	NULL		requires	NULL				ATP analogues	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_101	16030255	(E) Binding of myosin-Va by syntaxin-1A requires ATP analogues in presence of 10 - 6 M Ca2+.	bind
19775	3	5251	7	NULL	NULL	0	NULL	statement 2	NULL		occurs in presence of	NULL				Ca2+	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_101	16030255	(E) Binding of myosin-Va by syntaxin-1A requires ATP analogues in presence of 10 - 6 M Ca2+.	bind
14361	1	5252	6	NULL	NULL	NULL	NULL	Xpum	GP		bind			Puf		CPEB	GP				NULL		NULL	NULL	NULL	NULL	gw70_mechdev_120_8_865_s_90	12963108	(E) Binding of XPum Puf and  CPEB in immature	bind
15597	1	5252	7	NULL	NULL	0	NULL	XPum	NULL		bind	NULL		 Puf		CPEB	NULL				NULL		NULL	NULL	NULL	NULL	gw70_mechdev_120_8_865_s_90	12963108	(E) Binding of XPum Puf and  CPEB in immature	bind
14362	1	5253	6	NULL	NULL	NULL	NULL	APP	GP		bind		directly	C terminus		KLC1	GP		TPR domain		NULL		NULL	NULL	NULL	NULL	gw60_neuron_28_2_449_s_140	11144355	(E) C terminus of APP directly binds the TPR domain of KLC1.	bind
15134	1	5253	7	NULL	NULL	0	NULL	APP	NULL		binds	NULL	directly	C terminus		KLC1	NULL		TPR		NULL		0	NULL	NULL	NULL	gw60_neuron_28_2_449_s_140	11144355	(E) C terminus of APP directly binds the TPR domain of KLC1.	bind
14363	2	5254	6	NULL	NULL	NULL	NULL	C/EBP	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_113_4_495_s_194	12757710	(E) C/EBP  binds to E2F consensus within the DHFR promoter.	bind
53058	1	5254	6	NULL	NULL	NULL	NULL	E2F consensus	NucleicAcid		resides within					DHFR	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_cell_113_4_495_s_194	12757710	(E) C/EBP  binds to E2F consensus within the DHFR promoter.	bind
15135	2	5254	7	10	NULL	0	NULL	C/EBP	NULL		binds	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cell_113_4_495_s_194	12757710	(E) C/EBP  binds to E2F consensus within the DHFR promoter.	bind
53059	1	5254	7	10	NULL	0	NULL	E2F consensus	NULL		resides within	NULL				DHFR	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_cell_113_4_495_s_194	12757710	(E) C/EBP  binds to E2F consensus within the DHFR promoter.	bind
14364	1	5255	6	NULL	NULL	NULL	NULL	His6 - syntaxin 1 	GP		bind					GST-syncollin	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_cell_90_2_325_s_147	9244306	(E) Ca2+ sensitivity of  the binding of His6 - syntaxin 1 to GST-syncollinshort, immobilized on glutathione - agarose.	bind
53060	2	5255	6	NULL	NULL	NULL	NULL	statement 1	Process		is sensitive to					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_90_2_325_s_147	9244306	(E) Ca2+ sensitivity of  the binding of His6 - syntaxin 1 to GST-syncollinshort, immobilized on glutathione - agarose.	bind
15136	1	5255	7	NULL	NULL	0	NULL	His6 - syntaxin 1	NULL		bind	NULL				GST-syncollinshort	NULL	immobilized			NULL		0	NULL	NULL	NULL	gw60_cell_90_2_325_s_147	9244306	(E) Ca2+ sensitivity of  the binding of His6 - syntaxin 1 to GST-syncollinshort, immobilized on glutathione - agarose.	bind
15137	2	5255	7	NULL	NULL	0	NULL	statement 1	NULL		is sensitive to	NULL				Ca2+	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_90_2_325_s_147	9244306	(E) Ca2+ sensitivity of  the binding of His6 - syntaxin 1 to GST-syncollinshort, immobilized on glutathione - agarose.	bind
14365	1	5256	6	NULL	NULL	NULL	NULL	Cdc42p	GP	wild type	bind					Ste20p	GP		CRIB domain		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_6_2824_s_308	16571678	(E) Cdc42[V36]p GTPgammaS binds the Ste20p CRIB domain similar to wild-type Cdc42p.	bind
14366	2	5256	6	NULL	NULL	NULL	NULL	Cdc42[V36]p GTPgammaS	GP		bind					Ste20p	GP		CRIB domain		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_6_2824_s_308	16571678	(E) Cdc42[V36]p GTPgammaS binds the Ste20p CRIB domain similar to wild-type Cdc42p.	bind
15138	1	5256	7	NULL	NULL	0	NULL	Cdc42[V36]p GTPgammaS	NULL		bind	NULL				Ste20p	NULL		CRIB 		NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_6_2824_s_308	16571678	(E) Cdc42[V36]p GTPgammaS binds the Ste20p CRIB domain similar to wild-type Cdc42p.	bind
15139	2	5256	7	NULL	NULL	0	NULL	Cdc42p 	NULL	wild-type	bind	NULL				Ste20p	NULL		CRIB		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_6_2824_s_308	16571678	(E) Cdc42[V36]p GTPgammaS binds the Ste20p CRIB domain similar to wild-type Cdc42p.	bind
14367	1	5258	6	NULL	NULL	NULL	NULL	E2F1	GP		bind					Rb	GP			promoter	NULL	E13.5 embryonic brain	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_12_4448_s_265	16738312	(E) ChIP analysis demonstrates that E2F1 and E2F4, as well  as acetylated histone H3 are bound to the  Rb and  Cdc2 promoters, but not to intron 3 of the  Rb gene in the E13.5 embryonic brain.	bind
14368	2	5258	6	NULL	NULL	NULL	NULL	E2F1	GP		bind					cdc2	GP			promoter	NULL	E13.5 embryonic brain	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_12_4448_s_265	16738312	(E) ChIP analysis demonstrates that E2F1 and E2F4, as well  as acetylated histone H3 are bound to the  Rb and  Cdc2 promoters, but not to intron 3 of the  Rb gene in the E13.5 embryonic brain.	bind
14369	3	5258	6	NULL	NULL	NULL	NULL	histone H3	GP	acetylated	bind					Rb	GP			promoter	NULL	E13.5 embryonic brain	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_12_4448_s_265	16738312	(E) ChIP analysis demonstrates that E2F1 and E2F4, as well  as acetylated histone H3 are bound to the  Rb and  Cdc2 promoters, but not to intron 3 of the  Rb gene in the E13.5 embryonic brain.	bind
14370	4	5258	6	NULL	NULL	NULL	NULL	histone H3	GP	acetylated	bind					cdc42	GP			promoter	NULL	E13.5 embryonic brain	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_12_4448_s_265	16738312	(E) ChIP analysis demonstrates that E2F1 and E2F4, as well  as acetylated histone H3 are bound to the  Rb and  Cdc2 promoters, but not to intron 3 of the  Rb gene in the E13.5 embryonic brain.	bind
14371	5	5258	6	NULL	NULL	NULL	NULL	E2F4	GP		bind					Rb	GP			promoter	NULL	E13.5 embryonic brain	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_12_4448_s_265	16738312	(E) ChIP analysis demonstrates that E2F1 and E2F4, as well  as acetylated histone H3 are bound to the  Rb and  Cdc2 promoters, but not to intron 3 of the  Rb gene in the E13.5 embryonic brain.	bind
14372	6	5258	6	NULL	NULL	NULL	NULL	E2F4	GP		bind					Cdc2	GP			promoter	NULL	E13.5 embryonic brain	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_12_4448_s_265	16738312	(E) ChIP analysis demonstrates that E2F1 and E2F4, as well  as acetylated histone H3 are bound to the  Rb and  Cdc2 promoters, but not to intron 3 of the  Rb gene in the E13.5 embryonic brain.	bind
14373	7	5258	6	NULL	NULL	NULL	NULL	E2F1	GP		does not bind					Rb	GP			intron 3	NULL	E13.5 embryonic brain	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_12_4448_s_265	16738312	(E) ChIP analysis demonstrates that E2F1 and E2F4, as well  as acetylated histone H3 are bound to the  Rb and  Cdc2 promoters, but not to intron 3 of the  Rb gene in the E13.5 embryonic brain.	bind
14374	8	5258	6	NULL	NULL	NULL	NULL	E2F4	GP		does not bind					Rb	GP			intron 3	NULL	E13.5 embryonic brain	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_12_4448_s_265	16738312	(E) ChIP analysis demonstrates that E2F1 and E2F4, as well  as acetylated histone H3 are bound to the  Rb and  Cdc2 promoters, but not to intron 3 of the  Rb gene in the E13.5 embryonic brain.	bind
14375	9	5258	6	NULL	NULL	NULL	NULL	histone H3	GP	acetylated	bind					Rb	GP			intron 3	NULL	E13.5 embryonic brain	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_12_4448_s_265	16738312	(E) ChIP analysis demonstrates that E2F1 and E2F4, as well  as acetylated histone H3 are bound to the  Rb and  Cdc2 promoters, but not to intron 3 of the  Rb gene in the E13.5 embryonic brain.	bind
15141	1	5258	7	NULL	NULL	0	NULL	E2F1	NULL		bind	NULL				 Rb	NULL			promoter	NULL	E13.5 embryonic brain	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_12_4448_s_265	16738312	(E) ChIP analysis demonstrates that E2F1 and E2F4, as well  as acetylated histone H3 are bound to the  Rb and  Cdc2 promoters, but not to intron 3 of the  Rb gene in the E13.5 embryonic brain.	bind
15142	2	5258	7	NULL	NULL	0	NULL	E2F1	NULL		bind	NULL				Cdc2	NULL			promoter	NULL	E13.5 embryonic brain	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_12_4448_s_265	16738312	(E) ChIP analysis demonstrates that E2F1 and E2F4, as well  as acetylated histone H3 are bound to the  Rb and  Cdc2 promoters, but not to intron 3 of the  Rb gene in the E13.5 embryonic brain.	bind
15143	3	5258	7	NULL	NULL	0	NULL	E2F1	NULL		does not bind	NULL				Rb	NULL			 intron 3	NULL	E13.5 embryonic brain	0	NULL	NULL	NULL	gw70_molcellbiol_26_12_4448_s_265	16738312	(E) ChIP analysis demonstrates that E2F1 and E2F4, as well  as acetylated histone H3 are bound to the  Rb and  Cdc2 promoters, but not to intron 3 of the  Rb gene in the E13.5 embryonic brain.	bind
15144	4	5258	7	NULL	NULL	0	NULL	E2F4	NULL		bind	NULL				Rb	NULL			promoter	NULL	E13.5 embryonic brain	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_12_4448_s_265	16738312	(E) ChIP analysis demonstrates that E2F1 and E2F4, as well  as acetylated histone H3 are bound to the  Rb and  Cdc2 promoters, but not to intron 3 of the  Rb gene in the E13.5 embryonic brain.	bind
15145	5	5258	7	NULL	NULL	0	NULL	E2F4	NULL		bind	NULL				Cdc2	NULL			promoter	NULL	E13.5 embryonic brain	0	NULL	NULL	NULL	gw70_molcellbiol_26_12_4448_s_265	16738312	(E) ChIP analysis demonstrates that E2F1 and E2F4, as well  as acetylated histone H3 are bound to the  Rb and  Cdc2 promoters, but not to intron 3 of the  Rb gene in the E13.5 embryonic brain.	bind
15146	6	5258	7	NULL	NULL	0	NULL	E2F4	NULL		does not bind	NULL				Rb	NULL			intron 3	NULL	E13.5 embryonic brain	0	NULL	NULL	NULL	gw70_molcellbiol_26_12_4448_s_265	16738312	(E) ChIP analysis demonstrates that E2F1 and E2F4, as well  as acetylated histone H3 are bound to the  Rb and  Cdc2 promoters, but not to intron 3 of the  Rb gene in the E13.5 embryonic brain.	bind
15147	7	5258	7	NULL	NULL	0	NULL	histone H3	NULL	acetylated	bind	NULL				Rb	NULL			promoter	NULL	E13.5 embryonic brain	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_12_4448_s_265	16738312	(E) ChIP analysis demonstrates that E2F1 and E2F4, as well  as acetylated histone H3 are bound to the  Rb and  Cdc2 promoters, but not to intron 3 of the  Rb gene in the E13.5 embryonic brain.	bind
15148	8	5258	7	NULL	NULL	0	NULL	histone H3	NULL	acetylated	bind	NULL				Cdc2	NULL			promoter	NULL	E13.5 embryonic brain	0	NULL	NULL	NULL	gw70_molcellbiol_26_12_4448_s_265	16738312	(E) ChIP analysis demonstrates that E2F1 and E2F4, as well  as acetylated histone H3 are bound to the  Rb and  Cdc2 promoters, but not to intron 3 of the  Rb gene in the E13.5 embryonic brain.	bind
15149	9	5258	7	NULL	NULL	0	NULL	histone H3	NULL	acetylated	does not bind	NULL				Rb	NULL			intron 3	NULL	E13.5 embryonic brain	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_12_4448_s_265	16738312	(E) ChIP analysis demonstrates that E2F1 and E2F4, as well  as acetylated histone H3 are bound to the  Rb and  Cdc2 promoters, but not to intron 3 of the  Rb gene in the E13.5 embryonic brain.	bind
14376	1	5259	6	NULL	NULL	NULL	NULL	TBP	GP		bind					GAL1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_18_6270_s_218	11509669	(E) ChIP analysis of the binding of TBP to the  GAL1 and  GAL10 promoters.	bind
14377	2	5259	6	NULL	NULL	NULL	NULL	TBP	GP		bind					GAL10	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_18_6270_s_218	11509669	(E) ChIP analysis of the binding of TBP to the  GAL1 and  GAL10 promoters.	bind
15150	1	5259	7	NULL	NULL	0	NULL	TBP	NULL		bind	NULL				GAL1	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_18_6270_s_218	11509669	(E) ChIP analysis of the binding of TBP to the  GAL1 and  GAL10 promoters.	bind
15151	2	5259	7	NULL	NULL	0	NULL	TBP	NULL		bind	NULL				GAL10	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_18_6270_s_218	11509669	(E) ChIP analysis of the binding of TBP to the  GAL1 and  GAL10 promoters.	bind
14378	1	5260	6	NULL	NULL	NULL	NULL	H3	GP	methylated	bind			R17		TgCARM1	GP				NULL	extracellular tachyzoites treated with AMI-1	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10301_s_50	16287846	(E) ChIP experiments with extracellular tachyzoites treated with  AMI-1 or dimethyl sulfoxide (control) display the binding of methylated H3 [R17]  on TgCARM1 target  SAG1 and  SAG2A genes (Fig.  6A).	bind
14818	2	5260	6	NULL	NULL	NULL	NULL	H3	GP	methylated	bind			R17		TgCARM1	GP				NULL	extracellular tachyzoites treated with dimethyl sulfoxide	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10301_s_50	16287846	(E) ChIP experiments with extracellular tachyzoites treated with  AMI-1 or dimethyl sulfoxide (control) display the binding of methylated H3 [R17]  on TgCARM1 target  SAG1 and  SAG2A genes (Fig.  6A).	bind
14821	3	5260	6	NULL	NULL	NULL	NULL	statement 1	Process		target					SAG1 gene	GP				NULL	extracellular tachyzoites treated with AMI-1	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10301_s_50	16287846	(E) ChIP experiments with extracellular tachyzoites treated with  AMI-1 or dimethyl sulfoxide (control) display the binding of methylated H3 [R17]  on TgCARM1 target  SAG1 and  SAG2A genes (Fig.  6A).	bind
14822	4	5260	6	NULL	NULL	NULL	NULL	statement 1	Process		target					SAG2A gene	GP				NULL	extracellular tachyzoites treated with AMI-1	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10301_s_50	16287846	(E) ChIP experiments with extracellular tachyzoites treated with  AMI-1 or dimethyl sulfoxide (control) display the binding of methylated H3 [R17]  on TgCARM1 target  SAG1 and  SAG2A genes (Fig.  6A).	bind
16199	5	5260	6	NULL	NULL	NULL	NULL	statement 2	Process		target					SAG1 gene	GP				NULL	extracellular tachyzoites treated with AMI-1	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10301_s_50	16287846	(E) ChIP experiments with extracellular tachyzoites treated with  AMI-1 or dimethyl sulfoxide (control) display the binding of methylated H3 [R17]  on TgCARM1 target  SAG1 and  SAG2A genes (Fig.  6A).	bind
16200	6	5260	6	NULL	NULL	NULL	NULL	statement 2	Process		target					SAG2A gene	GP				NULL	extracellular tachyzoites treated with AMI-1	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10301_s_50	16287846	(E) ChIP experiments with extracellular tachyzoites treated with  AMI-1 or dimethyl sulfoxide (control) display the binding of methylated H3 [R17]  on TgCARM1 target  SAG1 and  SAG2A genes (Fig.  6A).	bind
15152	1	5260	7	NULL	NULL	0	NULL	H3 	NULL	methylated	bind	NULL		R17		TgCARM1	NULL			 	NULL	extracellular tachyzoites treated with  AMI-1	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10301_s_50	16287846	(E) ChIP experiments with extracellular tachyzoites treated with  AMI-1 or dimethyl sulfoxide (control) display the binding of methylated H3 [R17]  on TgCARM1 target  SAG1 and  SAG2A genes (Fig.  6A).	bind
15153	2	5260	7	NULL	NULL	0	NULL	H3 	NULL	methylated	bind	NULL		R17		TgCARM1	NULL				NULL	extracellular tachyzoites treated with  dimethyl sulfoxide	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10301_s_50	16287846	(E) ChIP experiments with extracellular tachyzoites treated with  AMI-1 or dimethyl sulfoxide (control) display the binding of methylated H3 [R17]  on TgCARM1 target  SAG1 and  SAG2A genes (Fig.  6A).	bind
15154	3	5260	7	10	NULL	0	NULL	statement 1	NULL		bind	NULL				SAG1 gene	NULL				NULL	extracellular tachyzoites treated with AMI-1	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10301_s_50	16287846	(E) ChIP experiments with extracellular tachyzoites treated with  AMI-1 or dimethyl sulfoxide (control) display the binding of methylated H3 [R17]  on TgCARM1 target  SAG1 and  SAG2A genes (Fig.  6A).	bind
15155	4	5260	7	10	NULL	0	NULL	statement 2	NULL		bind	NULL				SAG1 gene	NULL				NULL	extracellular tachyzoites treated with AMI-1	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10301_s_50	16287846	(E) ChIP experiments with extracellular tachyzoites treated with  AMI-1 or dimethyl sulfoxide (control) display the binding of methylated H3 [R17]  on TgCARM1 target  SAG1 and  SAG2A genes (Fig.  6A).	bind
15595	5	5260	7	10	NULL	0	NULL	statement 1	NULL		bind	NULL				SAG2A gene	NULL				NULL	extracellular tachyzoites treated with AMI-1	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10301_s_50	16287846	(E) ChIP experiments with extracellular tachyzoites treated with  AMI-1 or dimethyl sulfoxide (control) display the binding of methylated H3 [R17]  on TgCARM1 target  SAG1 and  SAG2A genes (Fig.  6A).	bind
15596	6	5260	7	10	NULL	0	NULL	statement 2	NULL		bind	NULL				SAG2A gene	NULL				NULL	extracellular tachyzoites treated with AMI-1	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10301_s_50	16287846	(E) ChIP experiments with extracellular tachyzoites treated with  AMI-1 or dimethyl sulfoxide (control) display the binding of methylated H3 [R17]  on TgCARM1 target  SAG1 and  SAG2A genes (Fig.  6A).	bind
14379	1	5261	6	NULL	NULL	NULL	NULL	TAp73alpha	GP		bind					p21	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_24_10593_s_397	15572666	(E) ChIP with  anti-HA antibodies in cells overexpressing HA-TAp73alpha alone or in combination with PIAS-1 or PIAS-1 and SUMO-1, showing reduced binding  of TAp73alpha to the p21 promoter in the presence of PIAS-1.	bind
14380	2	5261	6	NULL	NULL	NULL	NULL	statement 1	Process		is reduced in					PIAS-1	GP	presence of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_24_10593_s_397	15572666	(E) ChIP with  anti-HA antibodies in cells overexpressing HA-TAp73alpha alone or in combination with PIAS-1 or PIAS-1 and SUMO-1, showing reduced binding  of TAp73alpha to the p21 promoter in the presence of PIAS-1.	bind
15156	1	5261	7	NULL	NULL	0	NULL	TAp73alpha 	NULL		binding 	NULL				p21	NULL			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_24_10593_s_397	15572666	(E) ChIP with  anti-HA antibodies in cells overexpressing HA-TAp73alpha alone or in combination with PIAS-1 or PIAS-1 and SUMO-1, showing reduced binding  of TAp73alpha to the p21 promoter in the presence of PIAS-1.	bind
15598	2	5261	7	10	NULL	0	NULL	statement 1	NULL		is reduced in	NULL				PIAS-1	NULL	presence of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_24_10593_s_397	15572666	(E) ChIP with  anti-HA antibodies in cells overexpressing HA-TAp73alpha alone or in combination with PIAS-1 or PIAS-1 and SUMO-1, showing reduced binding  of TAp73alpha to the p21 promoter in the presence of PIAS-1.	bind
14381	1	5262	6	NULL	NULL	NULL	NULL	CLOCK	GP		bind					mPer1	GP			E box	NULL	circadian cycle	NULL	NULL	NULL	NULL	gw60_cell_107_7_855_s_168	11779462	(E) CLOCK and  BMAL1 are bound to the  mPer1 E  box over the circadian cycle.	bind
14382	2	5262	6	NULL	NULL	NULL	NULL	BMAL1	GP		bind					mPer1	GP			E box	NULL	circadian cycle	NULL	NULL	NULL	NULL	gw60_cell_107_7_855_s_168	11779462	(E) CLOCK and  BMAL1 are bound to the  mPer1 E  box over the circadian cycle.	bind
15157	1	5262	7	NULL	NULL	0	NULL	CLOCK 	NULL		bind	NULL				mPer1 	NULL			E box	NULL	circadian cycle	NULL	NULL	NULL	NULL	gw60_cell_107_7_855_s_168	11779462	(E) CLOCK and  BMAL1 are bound to the  mPer1 E  box over the circadian cycle.	bind
15158	2	5262	7	NULL	NULL	0	NULL	BMAL1	NULL		bind	NULL				mPer1 	NULL			E box 	NULL	circadian cycle	NULL	NULL	NULL	NULL	gw60_cell_107_7_855_s_168	11779462	(E) CLOCK and  BMAL1 are bound to the  mPer1 E  box over the circadian cycle.	bind
14383	1	5263	6	NULL	NULL	NULL	NULL	GST-CNP	GP		bind					MTs	CellComponent	preassembled			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_170_4_661_s_74	16103231	(E) Comparison of CNP and tau binding to MTs. Different amounts of GST-CNP (left) and tau (right) were cosedimented with preassembled MTs and analyzed by immunoblotting.	bind
14384	2	5263	6	NULL	NULL	NULL	NULL	tau	GP		bind					MTs	CellComponent	preassembled			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_170_4_661_s_74	16103231	(E) Comparison of CNP and tau binding to MTs. Different amounts of GST-CNP (left) and tau (right) were cosedimented with preassembled MTs and analyzed by immunoblotting.	bind
15159	1	5263	7	10	NULL	0	NULL	GST-CNP	NULL		bind	NULL				MTs	NULL	preassembled			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_170_4_661_s_74	16103231	(E) Comparison of CNP and tau binding to MTs. Different amounts of GST-CNP (left) and tau (right) were cosedimented with preassembled MTs and analyzed by immunoblotting.	bind
15160	2	5263	7	10	NULL	0	NULL	tau	NULL		bind	NULL				MTs	NULL	preassembled			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_170_4_661_s_74	16103231	(E) Comparison of CNP and tau binding to MTs. Different amounts of GST-CNP (left) and tau (right) were cosedimented with preassembled MTs and analyzed by immunoblotting.	bind
14385	1	5264	6	NULL	NULL	NULL	NULL	Arr2	GP		bind					PIP3 resin	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_39_1_121_s_94	12848937	(E) Competition of Arr2 binding to the PIP3 resin with various concentrations of PIP3 and IP6 as indicated.	bind
14386	2	5264	6	NULL	NULL	NULL	NULL	PIP3	GP		bind					PIP3 resin	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_39_1_121_s_94	12848937	(E) Competition of Arr2 binding to the PIP3 resin with various concentrations of PIP3 and IP6 as indicated.	bind
14387	3	5264	6	NULL	NULL	NULL	NULL	statement 1	Process		competes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_39_1_121_s_94	12848937	(E) Competition of Arr2 binding to the PIP3 resin with various concentrations of PIP3 and IP6 as indicated.	bind
14388	4	5264	6	NULL	NULL	NULL	NULL	IP6	GP		bind					PIP3 resin	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_39_1_121_s_94	12848937	(E) Competition of Arr2 binding to the PIP3 resin with various concentrations of PIP3 and IP6 as indicated.	bind
14389	5	5264	6	NULL	NULL	NULL	NULL	statement 1	Process		competes					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_39_1_121_s_94	12848937	(E) Competition of Arr2 binding to the PIP3 resin with various concentrations of PIP3 and IP6 as indicated.	bind
15161	1	5264	7	NULL	NULL	0	NULL	Arr2	NULL		bind	NULL				 PIP3 resin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuron_39_1_121_s_94	12848937	(E) Competition of Arr2 binding to the PIP3 resin with various concentrations of PIP3 and IP6 as indicated.	bind
15162	2	5264	7	NULL	NULL	0	NULL	PIP3	NULL		bind	NULL				PIP3 resin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuron_39_1_121_s_94	12848937	(E) Competition of Arr2 binding to the PIP3 resin with various concentrations of PIP3 and IP6 as indicated.	bind
44723	3	5264	7	NULL	NULL	0	NULL	 IP6	NULL		bind	NULL				PIP3 resin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuron_39_1_121_s_94	12848937	(E) Competition of Arr2 binding to the PIP3 resin with various concentrations of PIP3 and IP6 as indicated.	bind
44724	4	5264	7	NULL	NULL	0	NULL	statement 1	NULL		compete with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_39_1_121_s_94	12848937	(E) Competition of Arr2 binding to the PIP3 resin with various concentrations of PIP3 and IP6 as indicated.	bind
44725	5	5264	7	NULL	NULL	0	NULL	statement 1	NULL		compete with	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_39_1_121_s_94	12848937	(E) Competition of Arr2 binding to the PIP3 resin with various concentrations of PIP3 and IP6 as indicated.	bind
14390	1	5265	6	NULL	NULL	NULL	NULL	Crt1	GP		bind					Ssn6-Tup1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_cell_94_5_595_s_59	9741624	(E) Crt1 binds Ssn6-Tup1 in vitro.	bind
15163	1	5265	7	NULL	NULL	0	NULL	Crt1	NULL		binds	NULL				Ssn6-Tup1	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_cell_94_5_595_s_59	9741624	(E) Crt1 binds Ssn6-Tup1 in vitro.	bind
14391	1	5266	6	NULL	NULL	NULL	NULL	PRA1	GP		bind					Pic-Zn1	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_25_1_203_s_172	10707984	(E) Detergent sensitivity of PRA1 binding to Pic-Zn1 in 0.01% Triton X-100 (closed squares), 0.05% Triton X-100 (open circles), 0.1% Triton X-100 (closed triangles), and 0.5% Triton X-100 (open diamonds).	bind
15164	1	5266	7	NULL	NULL	0	NULL	PRA1	NULL		bind	NULL				Pic-Zn1	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_25_1_203_s_172	10707984	(E) Detergent sensitivity of PRA1 binding to Pic-Zn1 in 0.01% Triton X-100 (closed squares), 0.05% Triton X-100 (open circles), 0.1% Triton X-100 (closed triangles), and 0.5% Triton X-100 (open diamonds).	bind
14392	1	5267	6	NULL	NULL	NULL	NULL	cyclin D1	GP		bind		directly			ER	GP		EF-region		NULL		NULL	NULL	NULL	NULL	gw60_cell_88_3_405_s_217	9039267	(E) Direct binding between cyclin D1 and EF-region of  ER.	bind
15165	1	5267	7	NULL	NULL	0	NULL	cyclin D1	NULL		binds	NULL	directly			ER	NULL		EF region		NULL		0	NULL	NULL	NULL	gw60_cell_88_3_405_s_217	9039267	(E) Direct binding between cyclin D1 and EF-region of  ER.	bind
14393	1	5268	6	NULL	NULL	NULL	NULL	Grb2	GP		bind		directly			FRS2	GP				NULL	FGF-stimulated cells	NULL	NULL	NULL	NULL	gw60_cell_89_5_693_s_43	9182757	(E) Direct binding of Grb2 to FRS2 in FGF-stimulated cells.	bind
15166	1	5268	7	NULL	NULL	0	NULL	Grb2	NULL		binds	NULL	directly			 FRS2 	NULL				NULL	FGF-stimulated cells	0	NULL	NULL	NULL	gw60_cell_89_5_693_s_43	9182757	(E) Direct binding of Grb2 to FRS2 in FGF-stimulated cells.	bind
14394	1	5269	6	NULL	NULL	NULL	NULL	LRP5	GP		bind		directly			Wnt1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_2_303_s_166	11956231	(E) Direct binding of LRP5 to Wnt1 or Wnt4.	bind
14395	2	5269	6	NULL	NULL	NULL	NULL	LRP5	GP		bind		directly			Wnt4	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_2_303_s_166	11956231	(E) Direct binding of LRP5 to Wnt1 or Wnt4.	bind
14396	3	5269	6	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_2_303_s_166	11956231	(E) Direct binding of LRP5 to Wnt1 or Wnt4.	bind
15167	1	5269	7	NULL	NULL	0	NULL	LRP5	NULL		binds	NULL	directly			Wnt1	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_157_2_303_s_166	11956231	(E) Direct binding of LRP5 to Wnt1 or Wnt4.	bind
15168	2	5269	7	NULL	NULL	0	NULL	LRP5	NULL		binds	NULL	directly			Wnt4	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_157_2_303_s_166	11956231	(E) Direct binding of LRP5 to Wnt1 or Wnt4.	bind
15169	3	5269	7	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_157_2_303_s_166	11956231	(E) Direct binding of LRP5 to Wnt1 or Wnt4.	bind
14397	1	5270	6	NULL	NULL	NULL	NULL	TBP plus TFB	GP		bind									T1 BRE-TATA box sequences	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_187_18_6419_s_41	16159776	(E) DNase I footprints of the complexes formed by TBP  plus TFB binding to the T1, T2, and T3 BRE-TATA box sequences.	bind
14398	2	5270	6	NULL	NULL	NULL	NULL	TBP plus TFB	GP		bind									T2 BRE-TATA box sequences	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_187_18_6419_s_41	16159776	(E) DNase I footprints of the complexes formed by TBP  plus TFB binding to the T1, T2, and T3 BRE-TATA box sequences.	bind
14399	3	5270	6	NULL	NULL	NULL	NULL	TBP plus TFB	GP		bind									T3 BRE-TATA box sequences	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_187_18_6419_s_41	16159776	(E) DNase I footprints of the complexes formed by TBP  plus TFB binding to the T1, T2, and T3 BRE-TATA box sequences.	bind
15171	2	5270	7	NULL	NULL	0	NULL	TBP plus TFB	NULL		bind	NULL					NULL			 T1 BRE-TATA box sequences	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_187_18_6419_s_41	16159776	(E) DNase I footprints of the complexes formed by TBP  plus TFB binding to the T1, T2, and T3 BRE-TATA box sequences.	bind
15172	3	5270	7	NULL	NULL	0	NULL	TBP plus TFB	NULL		bind	NULL					NULL			T2 BRE-TATA box sequences	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_187_18_6419_s_41	16159776	(E) DNase I footprints of the complexes formed by TBP  plus TFB binding to the T1, T2, and T3 BRE-TATA box sequences.	bind
15173	4	5270	7	NULL	NULL	0	NULL	TBP plus TFB	NULL		bind	NULL					NULL			T3 BRE-TATA box sequences	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_187_18_6419_s_41	16159776	(E) DNase I footprints of the complexes formed by TBP  plus TFB binding to the T1, T2, and T3 BRE-TATA box sequences.	bind
14400	1	5272	6	NULL	NULL	NULL	NULL	Dock	GP		bind			SH3 domain		Dscam	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_cell_101_6_671_s_120	10892653	(E) Dock SH3 domains bind to Dscam  in vitro.	bind
15174	1	5272	7	NULL	NULL	0	NULL	Dock 	NULL		bind	NULL		SH3 domain		Dscam	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_cell_101_6_671_s_120	10892653	(E) Dock SH3 domains bind to Dscam  in vitro.	bind
14401	1	5273	6	NULL	NULL	NULL	NULL	RNAP	GP		bind					srf	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_12_4300_s_222	16740936	(E) Effect of  rpoA mutations on ComA-dependent RNAP binding to the  srf and  rpsD promoter and on Spx-dependent RNAP release from promoter DNA.	bind
14402	2	5273	6	NULL	NULL	NULL	NULL	RNAP	GP		bind					rpsD	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_12_4300_s_222	16740936	(E) Effect of  rpoA mutations on ComA-dependent RNAP binding to the  srf and  rpsD promoter and on Spx-dependent RNAP release from promoter DNA.	bind
14403	3	5273	6	NULL	NULL	NULL	NULL	statement 1	Process		is dependent on					ComA	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_12_4300_s_222	16740936	(E) Effect of  rpoA mutations on ComA-dependent RNAP binding to the  srf and  rpsD promoter and on Spx-dependent RNAP release from promoter DNA.	bind
14404	4	5273	6	NULL	NULL	NULL	NULL	statement 2	Process		is dependent on					ComA	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_12_4300_s_222	16740936	(E) Effect of  rpoA mutations on ComA-dependent RNAP binding to the  srf and  rpsD promoter and on Spx-dependent RNAP release from promoter DNA.	bind
14405	5	5273	6	NULL	NULL	NULL	NULL	DNA	NucleicAcid		release				promoter	RNAP	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_12_4300_s_222	16740936	(E) Effect of  rpoA mutations on ComA-dependent RNAP binding to the  srf and  rpsD promoter and on Spx-dependent RNAP release from promoter DNA.	bind
14406	6	5273	6	NULL	NULL	NULL	NULL	statement 5	Process		is dependent on					Spx	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_12_4300_s_222	16740936	(E) Effect of  rpoA mutations on ComA-dependent RNAP binding to the  srf and  rpsD promoter and on Spx-dependent RNAP release from promoter DNA.	bind
15175	1	5273	7	10	NULL	0	NULL	RNAP	NULL		bind	NULL				srf 	NULL			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_12_4300_s_222	16740936	(E) Effect of  rpoA mutations on ComA-dependent RNAP binding to the  srf and  rpsD promoter and on Spx-dependent RNAP release from promoter DNA.	bind
15176	2	5273	7	10	NULL	0	NULL	RNAP	NULL		bind	NULL				rpsD	NULL			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_12_4300_s_222	16740936	(E) Effect of  rpoA mutations on ComA-dependent RNAP binding to the  srf and  rpsD promoter and on Spx-dependent RNAP release from promoter DNA.	bind
15177	3	5273	7	10	NULL	0	NULL	RNAP	NULL		is release from	NULL				DNA	NULL			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_12_4300_s_222	16740936	(E) Effect of  rpoA mutations on ComA-dependent RNAP binding to the  srf and  rpsD promoter and on Spx-dependent RNAP release from promoter DNA.	bind
53061	4	5273	7	10	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				ComA	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_12_4300_s_222	16740936	(E) Effect of  rpoA mutations on ComA-dependent RNAP binding to the  srf and  rpsD promoter and on Spx-dependent RNAP release from promoter DNA.	bind
53062	5	5273	7	10	NULL	0	NULL	statement 2	NULL		is dependent on	NULL				ComA	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_12_4300_s_222	16740936	(E) Effect of  rpoA mutations on ComA-dependent RNAP binding to the  srf and  rpsD promoter and on Spx-dependent RNAP release from promoter DNA.	bind
53063	6	5273	7	10	NULL	0	NULL	statement 3	NULL		is dependent on	NULL				Spx	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_12_4300_s_222	16740936	(E) Effect of  rpoA mutations on ComA-dependent RNAP binding to the  srf and  rpsD promoter and on Spx-dependent RNAP release from promoter DNA.	bind
14407	1	5274	6	NULL	NULL	NULL	NULL	tau	GP		coimmunoprecipitates with					Fe65	GP				NULL	CGNs	NULL	NULL	NULL	NULL	gw70_neurobioldis_18_2_399_s_137	15686969	(E) Effect of the roscovitine (40  M) and lithium (10  M)  on the binding of Tau to Fe65 in CGNs. Immunoprecipitation and Western blot analysis  in B and E were performed as described in A. (E, F) Quantitative evaluation of the  effect of roscovitine and lithium on phosphorylation of tau at Tau-1 and AT8 sites  and their effect on the amount of tau co-immunoprecipitated with Fe65 (F).	bind
15205	1	5274	7	10	NULL	0	NULL	 Tau	NULL		coimmunoprecipitates with	NULL				Fe65 	NULL				NULL	CGNs	NULL	NULL	NULL	NULL	gw70_neurobioldis_18_2_399_s_137	15686969	(E) Effect of the roscovitine (40  M) and lithium (10  M)  on the binding of Tau to Fe65 in CGNs. Immunoprecipitation and Western blot analysis  in B and E were performed as described in A. (E, F) Quantitative evaluation of the  effect of roscovitine and lithium on phosphorylation of tau at Tau-1 and AT8 sites  and their effect on the amount of tau co-immunoprecipitated with Fe65 (F).	bind
14408	1	5275	6	NULL	NULL	NULL	NULL	Mgamma	GP		bind					B1 probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4600_s_156	10373509	(E) Effects of 5-, 10-, 20-, or 40-fold molar excess of either unlabeled A1 or A2 oligonucleotide on binding of Mgamma (50 ng) to the B1 probe.	bind
15178	1	5275	7	NULL	NULL	0	NULL	Mgamma	NULL		bind	NULL				B1 probe	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_7_4600_s_156	10373509	(E) Effects of 5-, 10-, 20-, or 40-fold molar excess of either unlabeled A1 or A2 oligonucleotide on binding of Mgamma (50 ng) to the B1 probe.	bind
14409	1	5276	6	NULL	NULL	NULL	NULL	CPSF	GP		bind					RNA	NucleicAcid	pre-wt			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2660_s_220	10733568	(E) Effects of DNA oligonucleotide competitors (Oligo) on the binding of CPSF to the pre-wt RNA.	bind
15179	1	5276	7	NULL	NULL	0	NULL	CPSF	NULL		bind	NULL				RNA	NULL	pre-wt			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_8_2660_s_220	10733568	(E) Effects of DNA oligonucleotide competitors (Oligo) on the binding of CPSF to the pre-wt RNA.	bind
14410	1	5277	6	NULL	NULL	NULL	NULL	CRT	GP		bind								DBD		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6286_s_238	12167720	(E) EGTA-sensitive binding of CRT to the DBD is partially lost on removal of the C-terminal domain (residues 1 to 273).	bind
14411	2	5277	6	NULL	NULL	NULL	NULL	statement 1	Process		is sensitive to					EGTA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6286_s_238	12167720	(E) EGTA-sensitive binding of CRT to the DBD is partially lost on removal of the C-terminal domain (residues 1 to 273).	bind
14412	3	5277	6	NULL	NULL	NULL	NULL	statement 1	Process		is lost upon		partially					removal of	C-terminal domain		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6286_s_238	12167720	(E) EGTA-sensitive binding of CRT to the DBD is partially lost on removal of the C-terminal domain (residues 1 to 273).	bind
15180	1	5277	7	10	NULL	0	NULL	 CRT	NULL		bind	NULL					NULL		DBD		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6286_s_238	12167720	(E) EGTA-sensitive binding of CRT to the DBD is partially lost on removal of the C-terminal domain (residues 1 to 273).	bind
15181	2	5277	7	NULL	NULL	0	NULL	statement 1	NULL		is sensitive to	NULL				EGTA	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6286_s_238	12167720	(E) EGTA-sensitive binding of CRT to the DBD is partially lost on removal of the C-terminal domain (residues 1 to 273).	bind
15182	3	5277	7	10	NULL	0	NULL	statement 1	NULL		is lost upon	NULL	partially				NULL	removal of 	C-terminal domain residues 1 to 273		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6286_s_238	12167720	(E) EGTA-sensitive binding of CRT to the DBD is partially lost on removal of the C-terminal domain (residues 1 to 273).	bind
14823	1	5278	6	NULL	NULL	NULL	NULL			deletion mutant	bind			delta1-4		SK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_3039_s_135	10082571	(E) EMSA carried out as described for panel D but performed at [[ 0 degrees C.                    The deletion mutants delta1-4 ]] and delta1-7 (Fig.  3A) both bound well to SK1 (Fig.  3B, lanes 8 and 9), and an EMSA titration indicated that delta1-7 and the Skn domain bound to this site with very similar affinities (Fig.  4A, lanes 1 to 10), indicating that the more distal (amino-terminal) residues in the arm (positions 1 to 7) (Fig.  3A) are not required for binding affinity.	bind
14824	2	5278	6	NULL	NULL	NULL	NULL			deletion mutant	bind			delta1-7		SK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_3039_s_135	10082571	(E) EMSA carried out as described for panel D but performed at [[ 0 degrees C.                    The deletion mutants delta1-4 ]] and delta1-7 (Fig.  3A) both bound well to SK1 (Fig.  3B, lanes 8 and 9), and an EMSA titration indicated that delta1-7 and the Skn domain bound to this site with very similar affinities (Fig.  4A, lanes 1 to 10), indicating that the more distal (amino-terminal) residues in the arm (positions 1 to 7) (Fig.  3A) are not required for binding affinity.	bind
53064	3	5278	6	NULL	NULL	NULL	NULL				is not required for			amino-terminal residues in the arm (1 to 7)		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_3039_s_135	10082571	(E) EMSA carried out as described for panel D but performed at [[ 0 degrees C.                    The deletion mutants delta1-4 ]] and delta1-7 (Fig.  3A) both bound well to SK1 (Fig.  3B, lanes 8 and 9), and an EMSA titration indicated that delta1-7 and the Skn domain bound to this site with very similar affinities (Fig.  4A, lanes 1 to 10), indicating that the more distal (amino-terminal) residues in the arm (positions 1 to 7) (Fig.  3A) are not required for binding affinity.	bind
15233	1	5278	7	NULL	NULL	0	NULL		NULL	deletion mutant	bind	NULL		delta1-4		SK1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_3039_s_135	10082571	(E) EMSA carried out as described for panel D but performed at [[ 0 degrees C.                    The deletion mutants delta1-4 ]] and delta1-7 (Fig.  3A) both bound well to SK1 (Fig.  3B, lanes 8 and 9), and an EMSA titration indicated that delta1-7 and the Skn domain bound to this site with very similar affinities (Fig.  4A, lanes 1 to 10), indicating that the more distal (amino-terminal) residues in the arm (positions 1 to 7) (Fig.  3A) are not required for binding affinity.	bind
15234	2	5278	7	NULL	NULL	0	NULL		NULL	deletion mutant	bind	NULL		delta1-7 		SK1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_3039_s_135	10082571	(E) EMSA carried out as described for panel D but performed at [[ 0 degrees C.                    The deletion mutants delta1-4 ]] and delta1-7 (Fig.  3A) both bound well to SK1 (Fig.  3B, lanes 8 and 9), and an EMSA titration indicated that delta1-7 and the Skn domain bound to this site with very similar affinities (Fig.  4A, lanes 1 to 10), indicating that the more distal (amino-terminal) residues in the arm (positions 1 to 7) (Fig.  3A) are not required for binding affinity.	bind
15235	3	5278	7	10	NULL	0	NULL		NULL		is not required for	NULL		amino-terminal residues in the arm (1 to 7)		statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_3039_s_135	10082571	(E) EMSA carried out as described for panel D but performed at [[ 0 degrees C.                    The deletion mutants delta1-4 ]] and delta1-7 (Fig.  3A) both bound well to SK1 (Fig.  3B, lanes 8 and 9), and an EMSA titration indicated that delta1-7 and the Skn domain bound to this site with very similar affinities (Fig.  4A, lanes 1 to 10), indicating that the more distal (amino-terminal) residues in the arm (positions 1 to 7) (Fig.  3A) are not required for binding affinity.	bind
14413	1	5279	6	NULL	NULL	NULL	NULL	HOX	GP		bind							wild type		40 bp oligonucleotide	NULL		NULL	NULL	NULL	NULL	gw70_devbiol_283_2_474_s_167	15913596	(E) EMSA of HOX and PBX1 binding to a 40-bp wild-type or mutant oligonucleotide  derived from 125 bp  Hb9 enhancer.	bind
14414	2	5279	6	NULL	NULL	NULL	NULL	HOX	GP		bind							mutant		40 bp oligonucleotide	NULL		NULL	NULL	NULL	NULL	gw70_devbiol_283_2_474_s_167	15913596	(E) EMSA of HOX and PBX1 binding to a 40-bp wild-type or mutant oligonucleotide  derived from 125 bp  Hb9 enhancer.	bind
14415	3	5279	6	NULL	NULL	NULL	NULL	PBX1	GP		bind							wild type		40 bp oligonucleotide	NULL		NULL	NULL	NULL	NULL	gw70_devbiol_283_2_474_s_167	15913596	(E) EMSA of HOX and PBX1 binding to a 40-bp wild-type or mutant oligonucleotide  derived from 125 bp  Hb9 enhancer.	bind
14416	4	5279	6	NULL	NULL	NULL	NULL	PBX1	GP		bind							mutant		40 bp oligonucleotide	NULL		NULL	NULL	NULL	NULL	gw70_devbiol_283_2_474_s_167	15913596	(E) EMSA of HOX and PBX1 binding to a 40-bp wild-type or mutant oligonucleotide  derived from 125 bp  Hb9 enhancer.	bind
54282	5	5279	6	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_283_2_474_s_167	15913596	(E) EMSA of HOX and PBX1 binding to a 40-bp wild-type or mutant oligonucleotide  derived from 125 bp  Hb9 enhancer.	bind
54283	6	5279	6	NULL	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_283_2_474_s_167	15913596	(E) EMSA of HOX and PBX1 binding to a 40-bp wild-type or mutant oligonucleotide  derived from 125 bp  Hb9 enhancer.	bind
54284	7	5279	6	NULL	NULL	NULL	NULL				is derived from				40 bp oligonucleotide	Hb9	GP			125 bp enhancer	NULL		NULL	NULL	NULL	NULL	gw70_devbiol_283_2_474_s_167	15913596	(E) EMSA of HOX and PBX1 binding to a 40-bp wild-type or mutant oligonucleotide  derived from 125 bp  Hb9 enhancer.	bind
15236	1	5279	7	NULL	NULL	0	NULL	HOX	NULL		bind	NULL					NULL	wild-type		40-bp oligonucleotide	NULL		0	NULL	NULL	NULL	gw70_devbiol_283_2_474_s_167	15913596	(E) EMSA of HOX and PBX1 binding to a 40-bp wild-type or mutant oligonucleotide  derived from 125 bp  Hb9 enhancer.	bind
15237	2	5279	7	NULL	NULL	0	NULL	HOX	NULL		bind	NULL					NULL	mutant		40-bp oligonucleotide	NULL		0	NULL	NULL	NULL	gw70_devbiol_283_2_474_s_167	15913596	(E) EMSA of HOX and PBX1 binding to a 40-bp wild-type or mutant oligonucleotide  derived from 125 bp  Hb9 enhancer.	bind
15238	3	5279	7	NULL	NULL	0	NULL	PBX1	NULL		bind	NULL					NULL	wild-type		40-bp oligonucleotide	NULL		0	NULL	NULL	NULL	gw70_devbiol_283_2_474_s_167	15913596	(E) EMSA of HOX and PBX1 binding to a 40-bp wild-type or mutant oligonucleotide  derived from 125 bp  Hb9 enhancer.	bind
15239	4	5279	7	NULL	NULL	0	NULL	PBX1	NULL		bind	NULL					NULL	mutant		40-bp oligonucleotide	NULL		0	NULL	NULL	NULL	gw70_devbiol_283_2_474_s_167	15913596	(E) EMSA of HOX and PBX1 binding to a 40-bp wild-type or mutant oligonucleotide  derived from 125 bp  Hb9 enhancer.	bind
15240	5	5279	7	NULL	NULL	0	NULL		NULL		is derived from	NULL			40-bp oligonucleotide	Hb9 	NULL			125 bp enhancer	NULL		0	NULL	NULL	NULL	gw70_devbiol_283_2_474_s_167	15913596	(E) EMSA of HOX and PBX1 binding to a 40-bp wild-type or mutant oligonucleotide  derived from 125 bp  Hb9 enhancer.	bind
15241	6	5279	7	NULL	NULL	0	NULL		NULL	mutant	is derived from	NULL			40-bp oligonucleotide	Hb9 	NULL			125 bp enhancer	NULL		0	NULL	NULL	NULL	gw70_devbiol_283_2_474_s_167	15913596	(E) EMSA of HOX and PBX1 binding to a 40-bp wild-type or mutant oligonucleotide  derived from 125 bp  Hb9 enhancer.	bind
15242	7	5279	7	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_283_2_474_s_167	15913596	(E) EMSA of HOX and PBX1 binding to a 40-bp wild-type or mutant oligonucleotide  derived from 125 bp  Hb9 enhancer.	bind
15243	8	5279	7	NULL	NULL	0	NULL	statement 3	NULL		is an alternative to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_283_2_474_s_167	15913596	(E) EMSA of HOX and PBX1 binding to a 40-bp wild-type or mutant oligonucleotide  derived from 125 bp  Hb9 enhancer.	bind
14601	1	5282	6	NULL	NULL	NULL	NULL	Miz-1	GP		bind					p21Cip1	GP			start site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_3_509_s_196	12408820	(E) Gel shift assays documenting binding of Miz-1 and TopBP1 to the start site of the  p21Cip1 promoter.	bind
14602	2	5282	6	NULL	NULL	NULL	NULL	TopBP1	GP		bind					p21Cip1	GP			start site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_3_509_s_196	12408820	(E) Gel shift assays documenting binding of Miz-1 and TopBP1 to the start site of the  p21Cip1 promoter.	bind
15244	1	5282	7	NULL	NULL	0	NULL	Miz-1 	NULL		bind	NULL				p21Cip1	NULL			start site of the promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_3_509_s_196	12408820	(E) Gel shift assays documenting binding of Miz-1 and TopBP1 to the start site of the  p21Cip1 promoter.	bind
15245	2	5282	7	NULL	NULL	0	NULL	TopBP1	NULL		bind	NULL				p21Cip1	NULL			start site of the promoter	NULL		0	NULL	NULL	NULL	gw60_molcell_10_3_509_s_196	12408820	(E) Gel shift assays documenting binding of Miz-1 and TopBP1 to the start site of the  p21Cip1 promoter.	bind
14603	1	5283	6	NULL	NULL	NULL	NULL	GST E1A 	GP		bind			C terminus		TnT CtBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_4_857_s_186	12419229	(E) GST E1A C  binding to TnT CtBP at various concentrations of NAD+, NADH, ADP-Ribose,  NMN, and Nicotinamide.	bind
15246	1	5283	7	NULL	NULL	0	NULL	GST E1A 	NULL		bind	NULL		C		TnT CtBP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_4_857_s_186	12419229	(E) GST E1A C  binding to TnT CtBP at various concentrations of NAD+, NADH, ADP-Ribose,  NMN, and Nicotinamide.	bind
14604	1	5286	6	NULL	NULL	NULL	NULL	hMSH2-hMSH6	GP		bind					DNA	NucleicAcid			b-GT	NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_2_255_s_36	10078208	(E) hMSH2-hMSH6 binding a  b-GT or  b-GC DNA in the presence or absence of MgCl2.	bind
14605	2	5286	6	NULL	NULL	NULL	NULL	hMSH2-hMSH6	GP		bind					DNA	NucleicAcid			b-GC	NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_2_255_s_36	10078208	(E) hMSH2-hMSH6 binding a  b-GT or  b-GC DNA in the presence or absence of MgCl2.	bind
15251	1	5286	7	NULL	NULL	0	NULL	hMSH2-hMSH6	NULL		bind	NULL				DNA	NULL			b-GT	NULL		0	NULL	NULL	NULL	gw60_molcell_3_2_255_s_36	10078208	(E) hMSH2-hMSH6 binding a  b-GT or  b-GC DNA in the presence or absence of MgCl2.	bind
15252	2	5286	7	NULL	NULL	0	NULL	hMSH2-hMSH6	NULL		bind	NULL				DNA	NULL			b-GC	NULL		0	NULL	NULL	NULL	gw60_molcell_3_2_255_s_36	10078208	(E) hMSH2-hMSH6 binding a  b-GT or  b-GC DNA in the presence or absence of MgCl2.	bind
14606	1	5287	6	NULL	NULL	NULL	NULL	HNF6	GP		bind					Glut2	GP			promoter	NULL	wild type liver chromatin	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7069_s_43	16055718	(e) HNF6 binds to  the Glut2 promoter in both wild-type and Foxa2-deficient liver chromatin, with a  trend towards less binding in the absence of Foxa2.	bind
14607	2	5287	6	NULL	NULL	NULL	NULL	HNF-6	GP		bind					Glut2	GP			promoter	NULL	Foxa2-deficient liver chromatin	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7069_s_43	16055718	(e) HNF6 binds to  the Glut2 promoter in both wild-type and Foxa2-deficient liver chromatin, with a  trend towards less binding in the absence of Foxa2.	bind
14608	3	5287	6	NULL	NULL	NULL	NULL	statement 2	Process		is less as compared to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7069_s_43	16055718	(e) HNF6 binds to  the Glut2 promoter in both wild-type and Foxa2-deficient liver chromatin, with a  trend towards less binding in the absence of Foxa2.	bind
15253	1	5287	7	NULL	NULL	0	NULL	HNF6 	NULL		binds	NULL				Glut2	NULL			promoter	NULL	 wild-type liver chromatin	0	NULL	NULL	NULL	gw70_molcellbiol_25_16_7069_s_43	16055718	(e) HNF6 binds to  the Glut2 promoter in both wild-type and Foxa2-deficient liver chromatin, with a  trend towards less binding in the absence of Foxa2.	bind
15254	2	5287	7	NULL	NULL	0	NULL	HNF6	NULL		binds	NULL				Glut2	NULL			promoter	NULL	Foxa2-deficient liver chromatin	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7069_s_43	16055718	(e) HNF6 binds to  the Glut2 promoter in both wild-type and Foxa2-deficient liver chromatin, with a  trend towards less binding in the absence of Foxa2.	bind
19987	4	5287	7	NULL	NULL	0	NULL	statement 2	NULL		is less than	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_16_7069_s_43	16055718	(e) HNF6 binds to  the Glut2 promoter in both wild-type and Foxa2-deficient liver chromatin, with a  trend towards less binding in the absence of Foxa2.	bind
14609	1	5288	6	NULL	NULL	NULL	NULL				bind		weakly	10C		MSL complexes	GP	partial			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_3_136_s_128	10679323	(e) Hoechst and (f) anti-Msl1 antibody staining pattern showing that 10C binds partial MSL complexes only weakly.	bind
15256	1	5288	7	NULL	NULL	0	NULL		NULL		binds	NULL	weakly	10C		MSL complexes	NULL	partial			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_3_136_s_128	10679323	(e) Hoechst and (f) anti-Msl1 antibody staining pattern showing that 10C binds partial MSL complexes only weakly.	bind
14610	1	5289	6	NULL	NULL	NULL	NULL	Rac1	GP	constitutively activated	bind					Pak	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_101_3_283_s_220	10847683	(E) In a yeast two-hybrid assay, constitutively activated Rac1  but not Mtl binds to Pak.	bind
14611	2	5289	6	NULL	NULL	NULL	NULL	Mtl	GP		does not bind					Pak	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_101_3_283_s_220	10847683	(E) In a yeast two-hybrid assay, constitutively activated Rac1  but not Mtl binds to Pak.	bind
15257	1	5289	7	NULL	NULL	0	NULL	Rac1	NULL	constitutively activated	binds to	NULL				Pak	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_101_3_283_s_220	10847683	(E) In a yeast two-hybrid assay, constitutively activated Rac1  but not Mtl binds to Pak.	bind
15258	2	5289	7	NULL	NULL	0	NULL	Mtl	NULL		does not bind	NULL				Pak	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_101_3_283_s_220	10847683	(E) In a yeast two-hybrid assay, constitutively activated Rac1  but not Mtl binds to Pak.	bind
14612	1	5290	6	NULL	NULL	NULL	NULL	Ras2	GP		bind					Lte1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_cellbiol_161_5_889_s_47	12782684	(e) In vitro binding of Ras2 and Lte1.	bind
15259	1	5290	7	NULL	NULL	0	NULL	Ras2	NULL		binds	NULL				Lte1	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_cellbiol_161_5_889_s_47	12782684	(e) In vitro binding of Ras2 and Lte1.	bind
14613	1	5291	6	NULL	NULL	NULL	NULL	ERK5	GP		induces					lklf gene	GP	endogenous			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8553_s_257	16166637	(E) Induction of the endogenous  lklf gene by ERK5.	bind
15260	1	5291	7	NULL	NULL	0	NULL	ERK5	NULL		induce	NULL				lklf gene	NULL	endogenous			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_19_8553_s_257	16166637	(E) Induction of the endogenous  lklf gene by ERK5.	bind
14614	1	5292	6	NULL	NULL	NULL	NULL	CIDR1alpha	GP		bind					B cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_9_5412_s_83	15322039	(E) Inhibition of CIDR1alpha binding to B cells with increasing concentrations of soluble IgG (upper panel) and  IgM (lower panel).	bind
14615	2	5292	6	NULL	NULL	NULL	NULL	IgG	GP	soluble	inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_9_5412_s_83	15322039	(E) Inhibition of CIDR1alpha binding to B cells with increasing concentrations of soluble IgG (upper panel) and  IgM (lower panel).	bind
14616	3	5292	6	NULL	NULL	NULL	NULL	IgM	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_72_9_5412_s_83	15322039	(E) Inhibition of CIDR1alpha binding to B cells with increasing concentrations of soluble IgG (upper panel) and  IgM (lower panel).	bind
15261	1	5292	7	NULL	NULL	0	NULL	CIDR1alpha	NULL		bind	NULL				B cells	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_72_9_5412_s_83	15322039	(E) Inhibition of CIDR1alpha binding to B cells with increasing concentrations of soluble IgG (upper panel) and  IgM (lower panel).	bind
15262	2	5292	7	NULL	NULL	0	NULL	 IgG	NULL	soluble	inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_72_9_5412_s_83	15322039	(E) Inhibition of CIDR1alpha binding to B cells with increasing concentrations of soluble IgG (upper panel) and  IgM (lower panel).	bind
15263	3	5292	7	NULL	NULL	0	NULL	IgM	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_72_9_5412_s_83	15322039	(E) Inhibition of CIDR1alpha binding to B cells with increasing concentrations of soluble IgG (upper panel) and  IgM (lower panel).	bind
14617	1	5293	6	NULL	NULL	NULL	NULL	FITC- E. coli	Organism		bind					dSR-CI	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_15_6_1027_s_165	11754822	(E) Inhibition profile of FITC- E. coli binding to dSR-CI.	bind
15264	1	5293	7	NULL	NULL	0	NULL	FITC- E. coli	NULL		bind	NULL				dSR-CI	NULL				NULL		0	NULL	NULL	NULL	gw60_immunity_15_6_1027_s_165	11754822	(E) Inhibition profile of FITC- E. coli binding to dSR-CI.	bind
14618	1	5294	6	NULL	NULL	NULL	NULL	Nck	GP		bind					CD3	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_109_7_901_s_213	12110186	(E) Interference with Nck binding to CD3  inhibits T cell proliferation.	bind
14619	2	5294	6	NULL	NULL	NULL	NULL	statement 1	Process	Interference with	inhibits					T cell	Cell	proliferation of			NULL		NULL	NULL	NULL	NULL	gw60_cell_109_7_901_s_213	12110186	(E) Interference with Nck binding to CD3  inhibits T cell proliferation.	bind
15265	1	5294	7	NULL	NULL	0	NULL	Nck	NULL		bind	NULL				CD3	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_109_7_901_s_213	12110186	(E) Interference with Nck binding to CD3  inhibits T cell proliferation.	bind
15266	2	5294	7	10	NULL	0	NULL	statement 1	NULL	interference with	inhibits	NULL				T cell	NULL	profileration of			NULL		NULL	NULL	NULL	NULL	gw60_cell_109_7_901_s_213	12110186	(E) Interference with Nck binding to CD3  inhibits T cell proliferation.	bind
14620	1	5296	6	NULL	NULL	NULL	NULL	MEK5	GP		bind			PB1 		ERK5	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_6_2065_s_114	16507987	(E) Mapping of residues  required for the MEK5 PB1 domain binding of ERK5.	bind
15267	1	5296	7	NULL	NULL	0	NULL	MEK5	NULL		bind	NULL		PB1 domain		ERK5	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_6_2065_s_114	16507987	(E) Mapping of residues  required for the MEK5 PB1 domain binding of ERK5.	bind
14621	1	5297	6	NULL	NULL	NULL	NULL	mDia1-N	GP		bind					GST-RhoA	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_13_15_1335_s_105	12906795	(E) mDia1-N binding to GST-RhoA.	bind
15268	1	5297	7	NULL	NULL	0	NULL	mDia1-N	NULL		bind	NULL				GST-RhoA	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_13_15_1335_s_105	12906795	(E) mDia1-N binding to GST-RhoA.	bind
14622	1	5298	6	NULL	NULL	NULL	NULL	Meox1	GP		bind		specifically			B7 oligonucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_7_2757_s_89	15024065	(E) Meox1 and Meox2 bound specifically to the B7 oligonucleotide.	bind
14623	2	5298	6	NULL	NULL	NULL	NULL	Meox2	GP		bind		specifically			B7 oligonucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_7_2757_s_89	15024065	(E) Meox1 and Meox2 bound specifically to the B7 oligonucleotide.	bind
15269	1	5298	7	NULL	NULL	0	NULL	Meox1	NULL		bind	NULL	specifically			B7 oligonucleotide	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_7_2757_s_89	15024065	(E) Meox1 and Meox2 bound specifically to the B7 oligonucleotide.	bind
15270	2	5298	7	NULL	NULL	0	NULL	Meox2	NULL		bind	NULL	specifically			B7 oligonucleotide	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_7_2757_s_89	15024065	(E) Meox1 and Meox2 bound specifically to the B7 oligonucleotide.	bind
14624	1	5299	6	NULL	NULL	NULL	NULL	Oct-3/4	GP		forms a complex with					Sox-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5453_s_225	10409735	(E) Model showing how the UTF1 regulatory element can selectively bind the complex comprising Oct-3/4 and Sox-2 and preclude the binding of Oct-6 together with Sox-2.	bind
14625	2	5299	6	NULL	NULL	NULL	NULL	UTF1	GP		bind		selectively		regulatory element	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5453_s_225	10409735	(E) Model showing how the UTF1 regulatory element can selectively bind the complex comprising Oct-3/4 and Sox-2 and preclude the binding of Oct-6 together with Sox-2.	bind
14626	3	5299	6	NULL	NULL	NULL	NULL	Oct-6	GP		bind					Sox-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5453_s_225	10409735	(E) Model showing how the UTF1 regulatory element can selectively bind the complex comprising Oct-3/4 and Sox-2 and preclude the binding of Oct-6 together with Sox-2.	bind
14627	4	5299	6	NULL	NULL	NULL	NULL	statement 2	Process		precludes					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5453_s_225	10409735	(E) Model showing how the UTF1 regulatory element can selectively bind the complex comprising Oct-3/4 and Sox-2 and preclude the binding of Oct-6 together with Sox-2.	bind
15271	1	5299	7	10	NULL	0	NULL	Oct-3/4	NULL		forms a complex with	NULL				Sox-2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5453_s_225	10409735	(E) Model showing how the UTF1 regulatory element can selectively bind the complex comprising Oct-3/4 and Sox-2 and preclude the binding of Oct-6 together with Sox-2.	bind
15272	2	5299	7	NULL	NULL	0	NULL	UTF1	NULL		bind	NULL	selectively		regulatory element	statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_8_5453_s_225	10409735	(E) Model showing how the UTF1 regulatory element can selectively bind the complex comprising Oct-3/4 and Sox-2 and preclude the binding of Oct-6 together with Sox-2.	bind
15273	3	5299	7	NULL	NULL	0	NULL	Oct-6	NULL		bind	NULL				Sox-2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_8_5453_s_225	10409735	(E) Model showing how the UTF1 regulatory element can selectively bind the complex comprising Oct-3/4 and Sox-2 and preclude the binding of Oct-6 together with Sox-2.	bind
15274	4	5299	7	10	NULL	0	NULL	statement 2	NULL		precludes	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5453_s_225	10409735	(E) Model showing how the UTF1 regulatory element can selectively bind the complex comprising Oct-3/4 and Sox-2 and preclude the binding of Oct-6 together with Sox-2.	bind
14628	1	5300	6	NULL	NULL	NULL	NULL	Monoclonal antibody AT8	GP		bind					PBs	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_308_3_646_s_77	12914799	(E) Monoclonal antibody AT8 (for hyperphosphorylated tau) bound to PBs and neuropil threads (arrow head).	bind
14629	2	5300	6	NULL	NULL	NULL	NULL	Monoclonal antibody AT8	GP		bind					neuropil threads	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_308_3_646_s_77	12914799	(E) Monoclonal antibody AT8 (for hyperphosphorylated tau) bound to PBs and neuropil threads (arrow head).	bind
15275	1	5300	7	10	NULL	0	NULL	Monoclonal antibody AT8	NULL		bind	NULL				PBs	NULL				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_308_3_646_s_77	12914799	(E) Monoclonal antibody AT8 (for hyperphosphorylated tau) bound to PBs and neuropil threads (arrow head).	bind
15276	2	5300	7	10	NULL	0	NULL	Monoclonal antibody AT8	NULL		bind	NULL				 neuropil threads	NULL				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_308_3_646_s_77	12914799	(E) Monoclonal antibody AT8 (for hyperphosphorylated tau) bound to PBs and neuropil threads (arrow head).	bind
14680	1	5301	5	10	NULL	0	NULL	p53		mutant	bind					Net					NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_3_1132_s_191	14729959	(E) Mutant p53s bind to Net. SAOS2 cells were transfected  with expression vectors for wild-type or mutant p53s and GST or GST-N6.	bind
14630	1	5301	6	NULL	NULL	NULL	NULL	p53	GP	mutant	bind					Net	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_3_1132_s_191	14729959	(E) Mutant p53s bind to Net. SAOS2 cells were transfected  with expression vectors for wild-type or mutant p53s and GST or GST-N6.	bind
14681	1	5302	5	NULL	NULL	0	NULL		NULL	newly translated	bind	NULL			G t		NULL			CCT	NULL	primary rat retinal culture	NULL	NULL	NULL	NULL	gw60_cell_89_6_927_s_92	9200611	(E) Newly translated G t in a primary rat  retinal culture becomes bound to CCT and is subsequently dissociated.	bind
14682	2	5302	5	NULL	NULL	0	NULL	statement 1	NULL		undergoes	NULL				dissociation	NULL	subsequent			NULL		0	NULL	NULL	NULL	gw60_cell_89_6_927_s_92	9200611	(E) Newly translated G t in a primary rat  retinal culture becomes bound to CCT and is subsequently dissociated.	bind
16208	1	5302	6	NULL	NULL	NULL	NULL	G t	GP	newly translated	bind									CCT	NULL	primary rat retinal culture	NULL	NULL	NULL	NULL	gw60_cell_89_6_927_s_92	9200611	(E) Newly translated G t in a primary rat  retinal culture becomes bound to CCT and is subsequently dissociated.	bind
16211	2	5302	6	NULL	NULL	NULL	NULL	G t	GP	newly translated	is dissociated from					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_89_6_927_s_92	9200611	(E) Newly translated G t in a primary rat  retinal culture becomes bound to CCT and is subsequently dissociated.	bind
14683	1	5303	5	NULL	NULL	0	NULL	p53	NULL		bind	NULL				IGFBP3	NULL			promoter	NULL	in vivo	0	NULL	NULL	NULL	gw70_molcellbiol_25_5_2014_s_357	15713654	(E) p53 and p53(deltaAD1deltaBD) bind the IGFBP3 promoter in vivo.	bind
14684	2	5303	5	NULL	NULL	0	NULL	p53	NULL		bind	NULL		deltaAD1deltaBD		IGFBP3	NULL			promoter	NULL	in vivo	0	NULL	NULL	NULL	gw70_molcellbiol_25_5_2014_s_357	15713654	(E) p53 and p53(deltaAD1deltaBD) bind the IGFBP3 promoter in vivo.	bind
14631	1	5303	6	NULL	NULL	NULL	NULL	p53	GP		bind					IGFBP3	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_2014_s_357	15713654	(E) p53 and p53(deltaAD1deltaBD) bind the IGFBP3 promoter in vivo.	bind
14632	2	5303	6	NULL	NULL	NULL	NULL	p53	GP		bind			deltaAD1deltaBD		IGFBP3	GP			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_2014_s_357	15713654	(E) p53 and p53(deltaAD1deltaBD) bind the IGFBP3 promoter in vivo.	bind
14685	1	5304	5	NULL	NULL	0	NULL	p53/6KR protein	NULL		bind	NULL				MDM2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_24_8533_s_228	11713288	(E) p53/6KR or 6KA protein binding to MDM2 was assessed as described in Materials and Methods.	bind
14686	2	5304	5	NULL	NULL	0	NULL	6KA protein	NULL		bind	NULL				MDM2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_24_8533_s_228	11713288	(E) p53/6KR or 6KA protein binding to MDM2 was assessed as described in Materials and Methods.	bind
14687	3	5304	5	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_24_8533_s_228	11713288	(E) p53/6KR or 6KA protein binding to MDM2 was assessed as described in Materials and Methods.	bind
14633	1	5304	6	NULL	NULL	NULL	NULL	p53/6KR protein	GP		bind					MDM2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_24_8533_s_228	11713288	(E) p53/6KR or 6KA protein binding to MDM2 was assessed as described in Materials and Methods.	bind
14634	2	5304	6	NULL	NULL	NULL	NULL	6KA protein	GP		bind					MDM2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_24_8533_s_228	11713288	(E) p53/6KR or 6KA protein binding to MDM2 was assessed as described in Materials and Methods.	bind
19020	3	5304	6	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_24_8533_s_228	11713288	(E) p53/6KR or 6KA protein binding to MDM2 was assessed as described in Materials and Methods.	bind
14688	1	5305	5	NULL	NULL	0	NULL	p54nrb	NULL		bind	NULL				I-RNA	NULL				NULL	in vivo	0	NULL	NULL	NULL	gw60_cell_106_4_465_s_225	11525732	(E) p54nrb binds I-RNA in vivo.	bind
14635	1	5305	6	NULL	NULL	NULL	NULL	p54nrb	GP		bind					I-RNA	NucleicAcid				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_cell_106_4_465_s_225	11525732	(E) p54nrb binds I-RNA in vivo.	bind
14689	1	5306	5	NULL	NULL	0	NULL	eIF4E	NULL		bind	NULL	selectively			cyclin D1	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_169_2_245_s_54	15837800	(E) Parallel  RT-PCR methods to the experiments in A - C confirm the above results indicating eIF4E  selectively binds cyclin D1 in a cap-dependent manner.	bind
14690	2	5306	5	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				cap	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_169_2_245_s_54	15837800	(E) Parallel  RT-PCR methods to the experiments in A - C confirm the above results indicating eIF4E  selectively binds cyclin D1 in a cap-dependent manner.	bind
14636	1	5306	6	NULL	NULL	NULL	NULL	eIF4E	GP		bind		selectively			cyclin D1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_169_2_245_s_54	15837800	(E) Parallel  RT-PCR methods to the experiments in A - C confirm the above results indicating eIF4E  selectively binds cyclin D1 in a cap-dependent manner.	bind
14637	2	5306	6	NULL	NULL	NULL	NULL	statement 1	Process		is dependent on					cap	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_169_2_245_s_54	15837800	(E) Parallel  RT-PCR methods to the experiments in A - C confirm the above results indicating eIF4E  selectively binds cyclin D1 in a cap-dependent manner.	bind
14691	1	5308	5	NULL	NULL	0	NULL	Phb-CC	NULL		bind	NULL				HDAC1	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_312_2_459_s_137	14637159	(E) Phb-CC  binds to HDAC1 in vitro.	bind
14638	1	5308	6	NULL	NULL	NULL	NULL	Phb-CC	GP		bind					HDAC1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_312_2_459_s_137	14637159	(E) Phb-CC  binds to HDAC1 in vitro.	bind
14692	1	5309	5	NULL	NULL	0	NULL	SMRT	NULL		associate with	NULL	physically			MEKK-1	NULL				NULL	in mammalian cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6612_s_258	10938135	(E) Physical association of SMRT with MEKK-1 and MEK-1 in mammalian cells.	bind
14693	2	5309	5	NULL	NULL	0	NULL	SMRT	NULL		associate with	NULL	physically			MEK-1	NULL				NULL	in mammalian cells	0	NULL	NULL	NULL	gw60_molcellbiol_20_17_6612_s_258	10938135	(E) Physical association of SMRT with MEKK-1 and MEK-1 in mammalian cells.	bind
14639	1	5309	6	NULL	NULL	NULL	NULL	SMRT	GP		associate with		physically			MEKK-1	GP				NULL	mammalian cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6612_s_258	10938135	(E) Physical association of SMRT with MEKK-1 and MEK-1 in mammalian cells.	bind
14640	2	5309	6	NULL	NULL	NULL	NULL	SMRT	GP		associate with		physically			MEK-1	GP				NULL	mammalian cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6612_s_258	10938135	(E) Physical association of SMRT with MEKK-1 and MEK-1 in mammalian cells.	bind
14752	1	5311	5	NULL	NULL	0	NULL	Ap-uch	NULL		bind	NULL				proteasome	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_89_1_115_s_177	9094720	(E) Quantification of Ap-uch bound to the proteasome (from blot  shown in panel D).	bind
14641	1	5311	6	NULL	NULL	NULL	NULL	Ap-uch	GP		bind					proteasome	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cell_89_1_115_s_177	9094720	(E) Quantification of Ap-uch bound to the proteasome (from blot  shown in panel D).	bind
14753	1	5312	5	NULL	NULL	0	NULL	TCF-4	NULL		bind	NULL				beta-catenin	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_154_2_369_s_254	11470825	(E) Quantification of the amount of TCF-4 bound to beta-catenin after 1alpha,25(OH)2D3 addition.	bind
14754	2	5312	5	NULL	NULL	0	NULL	statement 1	NULL		occurs after	NULL				1alpha,25(OH)2D3	NULL	addition of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_154_2_369_s_254	11470825	(E) Quantification of the amount of TCF-4 bound to beta-catenin after 1alpha,25(OH)2D3 addition.	bind
14642	1	5312	6	NULL	NULL	NULL	NULL	TCF-4	GP		bind					beta-catenin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_2_369_s_254	11470825	(E) Quantification of the amount of TCF-4 bound to beta-catenin after 1alpha,25(OH)2D3 addition.	bind
19021	2	5312	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs after 					1alpha,25(OH)2D3	Chemical	addition of			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_2_369_s_254	11470825	(E) Quantification of the amount of TCF-4 bound to beta-catenin after 1alpha,25(OH)2D3 addition.	bind
14756	1	5313	5	NULL	NULL	0	NULL	HDAC1	NULL		bind	NULL				bcl-2	NULL			P1 promoter	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_5_1608_s_287	15713621	(E) Quantitative ChIP assays of the binding of HDAC1 and HDAC2  to the  bcl-2 P1 promoter.	bind
14757	2	5313	5	NULL	NULL	0	NULL	HDAC2	NULL		bind	NULL				bcl-2	NULL			P1 promoter	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_5_1608_s_287	15713621	(E) Quantitative ChIP assays of the binding of HDAC1 and HDAC2  to the  bcl-2 P1 promoter.	bind
14643	1	5313	6	NULL	NULL	NULL	NULL	HDAC1	GP		bind					bcl-2 	GP			P1 promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1608_s_287	15713621	(E) Quantitative ChIP assays of the binding of HDAC1 and HDAC2  to the  bcl-2 P1 promoter.	bind
14644	2	5313	6	NULL	NULL	NULL	NULL	HDAC2	GP		bind					bcl-2 	GP			P1 promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1608_s_287	15713621	(E) Quantitative ChIP assays of the binding of HDAC1 and HDAC2  to the  bcl-2 P1 promoter.	bind
14758	1	5314	5	NULL	NULL	0	NULL	eIF4GI	NULL	recombinant	does not bind	NULL		(157-1090) Y776A		eIF4A	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_2_468_s_165	10611225	(E) Recombinant eIF4GI(157-1090) Y776A does not bind eIF4A.	bind
14645	1	5314	6	NULL	NULL	NULL	NULL	eIF4GI	GP	recombinant	does not bind			157-1090 Y776A		eIF4A	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_2_468_s_165	10611225	(E) Recombinant eIF4GI(157-1090) Y776A does not bind eIF4A.	bind
14759	1	5316	5	NULL	NULL	0	NULL		NULL		bind	NULL		PH domains		PI(3,4)P2	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_8_3242_s_172	12925760	(E) Residues   conserved in PH domains binding to PI(3,4)P2 and  PI(3,4,5)P3 (Isakoff  et  al., 1998 ) are aligned to the SWAP-70 sequence.	bind
14760	2	5316	5	NULL	NULL	0	NULL		NULL		bind	NULL		PH domains		PI(3,4,5)P3	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_8_3242_s_172	12925760	(E) Residues   conserved in PH domains binding to PI(3,4)P2 and  PI(3,4,5)P3 (Isakoff  et  al., 1998 ) are aligned to the SWAP-70 sequence.	bind
19022	1	5316	6	NULL	NULL	NULL	NULL				bind			PH domain		PI(3,4)P2	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_8_3242_s_172	12925760	(E) Residues   conserved in PH domains binding to PI(3,4)P2 and  PI(3,4,5)P3 (Isakoff  et  al., 1998 ) are aligned to the SWAP-70 sequence.	bind
19023	2	5316	6	NULL	NULL	NULL	NULL				bind			PH domain		PI(3,4,5)P3	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_8_3242_s_172	12925760	(E) Residues   conserved in PH domains binding to PI(3,4)P2 and  PI(3,4,5)P3 (Isakoff  et  al., 1998 ) are aligned to the SWAP-70 sequence.	bind
14763	1	5319	5	10	NULL	0	NULL	CUGBP2			bind		specifically							A-II region	NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_1_113_s_162	12535526	(E) Scanning mutagenesis identifies specific CUGBP2 binding to A-II and A-III regions.	bind
14764	2	5319	5	10	NULL	0	NULL	CUGBP2			bind		specifically							A-III region	NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_1_113_s_162	12535526	(E) Scanning mutagenesis identifies specific CUGBP2 binding to A-II and A-III regions.	bind
14646	1	5319	6	NULL	NULL	NULL	NULL	CUGBP2	GP		bind		specifically							A-II region	NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_1_113_s_162	12535526	(E) Scanning mutagenesis identifies specific CUGBP2 binding to A-II and A-III regions.	bind
14647	2	5319	6	NULL	NULL	NULL	NULL	CUGBP2	GP		bind		specifically							A-III region	NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_1_113_s_162	12535526	(E) Scanning mutagenesis identifies specific CUGBP2 binding to A-II and A-III regions.	bind
14766	1	5320	5	NULL	NULL	0	NULL	Sno	NULL		bind	NULL		C-terminal domain		Su(H)	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_110_5_625_s_257	12230979	(E) Sno binds to Su(H) via its C-terminal domain.	bind
14648	1	5320	6	NULL	NULL	NULL	NULL	Sno	GP		bind			C-terminal domain		Su(H)	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_110_5_625_s_257	12230979	(E) Sno binds to Su(H) via its C-terminal domain.	bind
14767	1	5321	5	NULL	NULL	0	NULL	dATF-2	NULL		bind	NULL	specifically				NULL			CRE	NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_6_2934_s_168	15788564	(E) Specific binding of  dATF-2 to CRE.	bind
14649	1	5321	6	NULL	NULL	NULL	NULL	dATF-2	GP		bind		specifically							CRE	NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_6_2934_s_168	15788564	(E) Specific binding of  dATF-2 to CRE.	bind
14769	1	5322	5	10	NULL	0	NULL	p53			bind		specifically			FAK				promoter	NULL	in HeLa cells	NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1678_2_111_s_344	15157737	(E) Specific binding of p53 with the FAK-promoter  probe in HeLa cells.	bind
14650	1	5322	6	NULL	NULL	NULL	NULL	p53	GP		bind		specifically			FAK	GP			promoter	NULL	HeLa cells	NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1678_2_111_s_344	15157737	(E) Specific binding of p53 with the FAK-promoter  probe in HeLa cells.	bind
14771	1	5323	5	NULL	NULL	0	NULL	FarB	NULL		bind	NULL				probe J7-8	NULL				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_5_5_794_s_239	16682457	(E) Specific competition of binding of FarB and FarA to probe J7-8.	bind
14772	2	5323	5	NULL	NULL	0	NULL	FarA	NULL		bind	NULL				probe J7-8	NULL				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_5_5_794_s_239	16682457	(E) Specific competition of binding of FarB and FarA to probe J7-8.	bind
14773	3	5323	5	NULL	NULL	0	NULL	statement 1	NULL		compete with	NULL	specifically			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_5_5_794_s_239	16682457	(E) Specific competition of binding of FarB and FarA to probe J7-8.	bind
14651	1	5323	6	NULL	NULL	NULL	NULL	FarB	GP		bind					probe J7-8	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_5_5_794_s_239	16682457	(E) Specific competition of binding of FarB and FarA to probe J7-8.	bind
14652	2	5323	6	NULL	NULL	NULL	NULL	FarA	GP		bind					probe J7-8	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_5_5_794_s_239	16682457	(E) Specific competition of binding of FarB and FarA to probe J7-8.	bind
19024	3	5323	6	NULL	NULL	NULL	NULL	statement 1	Process		competes		specifically			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_5_5_794_s_239	16682457	(E) Specific competition of binding of FarB and FarA to probe J7-8.	bind
14774	1	5325	5	NULL	NULL	0	NULL		NULL		bind	NULL		PDZ		CtBP1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_11_5_1389_s_153	12769861	(E) SUMOylation blocks PDZ binding to CtBP1.	bind
14775	2	5325	5	NULL	NULL	0	NULL	SUMOylation	NULL		blocks	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_11_5_1389_s_153	12769861	(E) SUMOylation blocks PDZ binding to CtBP1.	bind
14694	1	5325	6	NULL	NULL	NULL	NULL				bind			PDZ		CtBP1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_5_1389_s_153	12769861	(E) SUMOylation blocks PDZ binding to CtBP1.	bind
14695	2	5325	6	NULL	NULL	NULL	NULL	SUMOylation	Process		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_5_1389_s_153	12769861	(E) SUMOylation blocks PDZ binding to CtBP1.	bind
14776	1	5326	5	10	NULL	0	NULL	msl-2			bind				3 UTR 	SXL					NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_5_1397_s_78	12769862	(E) The 3  UTR  msl-2 sequences provide a function in addition to SXL binding.	bind
14696	1	5326	6	NULL	NULL	NULL	NULL	msl-2	GP		bind				3 UTR	SXL	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_5_1397_s_78	12769862	(E) The 3  UTR  msl-2 sequences provide a function in addition to SXL binding.	bind
14777	1	5328	5	NULL	NULL	0	NULL	p53	NULL		bind	NULL				p21	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_22_9958_s_144	15509798	(E) The effect of NAD or TDP on p53 binding  to p21 versus hdm2 DNA is quantified below each lane.	bind
14778	2	5328	5	NULL	NULL	0	NULL	p53	NULL		bind	NULL				hdm2 DNA	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_22_9958_s_144	15509798	(E) The effect of NAD or TDP on p53 binding  to p21 versus hdm2 DNA is quantified below each lane.	bind
14697	1	5328	6	NULL	NULL	NULL	NULL	p53	GP		bind					p21	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_22_9958_s_144	15509798	(E) The effect of NAD or TDP on p53 binding  to p21 versus hdm2 DNA is quantified below each lane.	bind
14698	2	5328	6	NULL	NULL	NULL	NULL	p53	GP		bind					hdm2 DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_22_9958_s_144	15509798	(E) The effect of NAD or TDP on p53 binding  to p21 versus hdm2 DNA is quantified below each lane.	bind
14779	1	5331	5	NULL	NULL	0	NULL	PLIC1	NULL		bind	NULL		UBA domain		K7	NULL				NULL	in 293T cells	0	NULL	NULL	NULL	gw70_molcellbiol_24_9_3938_s_133	15082787	(E) The PLIC1 UBA domain binds to K7 in 293T  cells.	bind
14699	1	5331	6	NULL	NULL	NULL	NULL	PLIC1	GP		bind			UBA		K7	GP				NULL	293T cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_9_3938_s_133	15082787	(E) The PLIC1 UBA domain binds to K7 in 293T  cells.	bind
14780	1	5332	5	NULL	NULL	0	NULL		NULL		bind	NULL		SH3 domains			NULL		DH domain		NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_4_1624_s_227	12686614	(E) The SH3 domains  bind the DH domain.	bind
14700	1	5332	6	NULL	NULL	NULL	NULL				bind			SH3 domain					DH domain		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_4_1624_s_227	12686614	(E) The SH3 domains  bind the DH domain.	bind
14781	1	5334	5	NULL	NULL	0	NULL	PBX	NULL		bind	NULL				CBP	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_21_7509_s_122	11585930	(E) The TALE motif does not prevent PBX binding to CBP, but changing an arginine to lysine within HD helix 3 increases CBP binding to PBX.	bind
14782	2	5334	5	NULL	NULL	0	NULL		NULL		does not prevent	NULL		TALE motif		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_21_7509_s_122	11585930	(E) The TALE motif does not prevent PBX binding to CBP, but changing an arginine to lysine within HD helix 3 increases CBP binding to PBX.	bind
14783	3	5334	5	NULL	NULL	0	NULL	arginine	NULL		changes to	NULL				lysine	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_21_7509_s_122	11585930	(E) The TALE motif does not prevent PBX binding to CBP, but changing an arginine to lysine within HD helix 3 increases CBP binding to PBX.	bind
19092	4	5334	5	NULL	NULL	0	NULL	statement 3	NULL		occurs in	NULL					NULL		HD helix 3		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_21_7509_s_122	11585930	(E) The TALE motif does not prevent PBX binding to CBP, but changing an arginine to lysine within HD helix 3 increases CBP binding to PBX.	bind
19093	5	5334	5	NULL	NULL	0	NULL	statement 4	NULL		increases	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_21_7509_s_122	11585930	(E) The TALE motif does not prevent PBX binding to CBP, but changing an arginine to lysine within HD helix 3 increases CBP binding to PBX.	bind
14701	1	5334	6	NULL	NULL	NULL	NULL	CBP	GP		bind					PBX	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_21_7509_s_122	11585930	(E) The TALE motif does not prevent PBX binding to CBP, but changing an arginine to lysine within HD helix 3 increases CBP binding to PBX.	bind
14702	2	5334	6	NULL	NULL	NULL	NULL				does not prevent			TALE motif		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_21_7509_s_122	11585930	(E) The TALE motif does not prevent PBX binding to CBP, but changing an arginine to lysine within HD helix 3 increases CBP binding to PBX.	bind
14703	3	5334	6	NULL	NULL	NULL	NULL	arginine	AminoAcid		changes to					lysine	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_21_7509_s_122	11585930	(E) The TALE motif does not prevent PBX binding to CBP, but changing an arginine to lysine within HD helix 3 increases CBP binding to PBX.	bind
19025	4	5334	6	NULL	NULL	NULL	NULL	statement 3	Process		occurs in								HD helix 3		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_21_7509_s_122	11585930	(E) The TALE motif does not prevent PBX binding to CBP, but changing an arginine to lysine within HD helix 3 increases CBP binding to PBX.	bind
19026	5	5334	6	NULL	NULL	NULL	NULL	statement 4	Process		increases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_21_7509_s_122	11585930	(E) The TALE motif does not prevent PBX binding to CBP, but changing an arginine to lysine within HD helix 3 increases CBP binding to PBX.	bind
14784	1	5337	5	NULL	NULL	0	NULL	iron	NULL		bind	NULL				Lf	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_21_6091_s_128	11029429	(e) Viable counts of  E. coli strain E2348/69 after 18 h of incubation from an inoculum of 102 CFU/ml in unsupplemented serum-SAPI medium (control) or in serum-SAPI medium supplemented with NE complexes of (i) the Tf isoform mixture used as markers in panel c above, (ii) Apo-Tf, (iii) iron-bound Lf, or (iv) BSA. (f) Binding of [3]NE, expressed as 3H cpm per 30 mug of protein, to (i) partially iron-saturated Tf, (ii) Apo-Tf, (iii) iron-bound Lf, or (iv) BSA; the values shown are the means of triplicate assays.	bind
14785	2	5337	5	10	NULL	0	NULL	NE			bind					Tf		partially iron-saturated			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_21_6091_s_128	11029429	(e) Viable counts of  E. coli strain E2348/69 after 18 h of incubation from an inoculum of 102 CFU/ml in unsupplemented serum-SAPI medium (control) or in serum-SAPI medium supplemented with NE complexes of (i) the Tf isoform mixture used as markers in panel c above, (ii) Apo-Tf, (iii) iron-bound Lf, or (iv) BSA. (f) Binding of [3]NE, expressed as 3H cpm per 30 mug of protein, to (i) partially iron-saturated Tf, (ii) Apo-Tf, (iii) iron-bound Lf, or (iv) BSA; the values shown are the means of triplicate assays.	bind
56060	3	5337	5	10	NULL	0	NULL	NE			bind					Apo-Tf					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_21_6091_s_128	11029429	(e) Viable counts of  E. coli strain E2348/69 after 18 h of incubation from an inoculum of 102 CFU/ml in unsupplemented serum-SAPI medium (control) or in serum-SAPI medium supplemented with NE complexes of (i) the Tf isoform mixture used as markers in panel c above, (ii) Apo-Tf, (iii) iron-bound Lf, or (iv) BSA. (f) Binding of [3]NE, expressed as 3H cpm per 30 mug of protein, to (i) partially iron-saturated Tf, (ii) Apo-Tf, (iii) iron-bound Lf, or (iv) BSA; the values shown are the means of triplicate assays.	bind
56061	4	5337	5	10	NULL	0	NULL	NE			bind					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_21_6091_s_128	11029429	(e) Viable counts of  E. coli strain E2348/69 after 18 h of incubation from an inoculum of 102 CFU/ml in unsupplemented serum-SAPI medium (control) or in serum-SAPI medium supplemented with NE complexes of (i) the Tf isoform mixture used as markers in panel c above, (ii) Apo-Tf, (iii) iron-bound Lf, or (iv) BSA. (f) Binding of [3]NE, expressed as 3H cpm per 30 mug of protein, to (i) partially iron-saturated Tf, (ii) Apo-Tf, (iii) iron-bound Lf, or (iv) BSA; the values shown are the means of triplicate assays.	bind
14704	1	5337	6	NULL	NULL	NULL	NULL	iron	Chemical		bind					Lf	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_21_6091_s_128	11029429	(e) Viable counts of  E. coli strain E2348/69 after 18 h of incubation from an inoculum of 102 CFU/ml in unsupplemented serum-SAPI medium (control) or in serum-SAPI medium supplemented with NE complexes of (i) the Tf isoform mixture used as markers in panel c above, (ii) Apo-Tf, (iii) iron-bound Lf, or (iv) BSA. (f) Binding of [3]NE, expressed as 3H cpm per 30 mug of protein, to (i) partially iron-saturated Tf, (ii) Apo-Tf, (iii) iron-bound Lf, or (iv) BSA; the values shown are the means of triplicate assays.	bind
19160	2	5337	6	NULL	NULL	NULL	NULL	NE	OrganismPart		bind					Tf	GP	partially iron-saturated			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_21_6091_s_128	11029429	(e) Viable counts of  E. coli strain E2348/69 after 18 h of incubation from an inoculum of 102 CFU/ml in unsupplemented serum-SAPI medium (control) or in serum-SAPI medium supplemented with NE complexes of (i) the Tf isoform mixture used as markers in panel c above, (ii) Apo-Tf, (iii) iron-bound Lf, or (iv) BSA. (f) Binding of [3]NE, expressed as 3H cpm per 30 mug of protein, to (i) partially iron-saturated Tf, (ii) Apo-Tf, (iii) iron-bound Lf, or (iv) BSA; the values shown are the means of triplicate assays.	bind
19161	3	5337	6	NULL	NULL	NULL	NULL	NE	OrganismPart		bind					Apo-Tf	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_21_6091_s_128	11029429	(e) Viable counts of  E. coli strain E2348/69 after 18 h of incubation from an inoculum of 102 CFU/ml in unsupplemented serum-SAPI medium (control) or in serum-SAPI medium supplemented with NE complexes of (i) the Tf isoform mixture used as markers in panel c above, (ii) Apo-Tf, (iii) iron-bound Lf, or (iv) BSA. (f) Binding of [3]NE, expressed as 3H cpm per 30 mug of protein, to (i) partially iron-saturated Tf, (ii) Apo-Tf, (iii) iron-bound Lf, or (iv) BSA; the values shown are the means of triplicate assays.	bind
19162	4	5337	6	NULL	NULL	NULL	NULL	NE	OrganismPart		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_21_6091_s_128	11029429	(e) Viable counts of  E. coli strain E2348/69 after 18 h of incubation from an inoculum of 102 CFU/ml in unsupplemented serum-SAPI medium (control) or in serum-SAPI medium supplemented with NE complexes of (i) the Tf isoform mixture used as markers in panel c above, (ii) Apo-Tf, (iii) iron-bound Lf, or (iv) BSA. (f) Binding of [3]NE, expressed as 3H cpm per 30 mug of protein, to (i) partially iron-saturated Tf, (ii) Apo-Tf, (iii) iron-bound Lf, or (iv) BSA; the values shown are the means of triplicate assays.	bind
14786	1	5338	5	NULL	NULL	0	NULL	Jacob	NULL	E. histolytica	bind	NULL				chitin	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_6_3259_s_40	12011021	(E) Western blot analysis of chitin binding by  E. histolytica Jacob, detected with anti-myc antibodies and chemiluminescence.	bind
14705	1	5338	6	NULL	NULL	NULL	NULL	Jacob	GP	E. histolytica	bind					chitin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_6_3259_s_40	12011021	(E) Western blot analysis of chitin binding by  E. histolytica Jacob, detected with anti-myc antibodies and chemiluminescence.	bind
14787	1	5339	5	NULL	NULL	0	NULL	Sam68	NULL		bind	NULL				cyclin B1	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_1_14_s_186	16221888	(E) Western blot analysis of the IgG, cyclin B1 and Erk1/2  immunoprecipitates from the kinase assay (D) probed with anti-Sam68 antibody: Sam68  binds both cyclin B1 and Erk1/2, but this interaction is inhibited by OA stimulation.	bind
14788	2	5339	5	NULL	NULL	0	NULL	Sam68	NULL		bind	NULL				Erk1/2	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_1_14_s_186	16221888	(E) Western blot analysis of the IgG, cyclin B1 and Erk1/2  immunoprecipitates from the kinase assay (D) probed with anti-Sam68 antibody: Sam68  binds both cyclin B1 and Erk1/2, but this interaction is inhibited by OA stimulation.	bind
14789	3	5339	5	NULL	NULL	0	NULL	OA	NULL	stimulation by	inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_1_14_s_186	16221888	(E) Western blot analysis of the IgG, cyclin B1 and Erk1/2  immunoprecipitates from the kinase assay (D) probed with anti-Sam68 antibody: Sam68  binds both cyclin B1 and Erk1/2, but this interaction is inhibited by OA stimulation.	bind
14790	4	5339	5	NULL	NULL	0	NULL	OA	NULL	stimulation by	inhibit	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_1_14_s_186	16221888	(E) Western blot analysis of the IgG, cyclin B1 and Erk1/2  immunoprecipitates from the kinase assay (D) probed with anti-Sam68 antibody: Sam68  binds both cyclin B1 and Erk1/2, but this interaction is inhibited by OA stimulation.	bind
14706	1	5339	6	NULL	NULL	NULL	NULL	Sam68	GP		bind					cyclin B1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_14_s_186	16221888	(E) Western blot analysis of the IgG, cyclin B1 and Erk1/2  immunoprecipitates from the kinase assay (D) probed with anti-Sam68 antibody: Sam68  binds both cyclin B1 and Erk1/2, but this interaction is inhibited by OA stimulation.	bind
14707	2	5339	6	NULL	NULL	NULL	NULL	Sam68	GP		bind					Erk1/2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_14_s_186	16221888	(E) Western blot analysis of the IgG, cyclin B1 and Erk1/2  immunoprecipitates from the kinase assay (D) probed with anti-Sam68 antibody: Sam68  binds both cyclin B1 and Erk1/2, but this interaction is inhibited by OA stimulation.	bind
14708	3	5339	6	NULL	NULL	NULL	NULL	OA	Chemical	stimulation of	inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_14_s_186	16221888	(E) Western blot analysis of the IgG, cyclin B1 and Erk1/2  immunoprecipitates from the kinase assay (D) probed with anti-Sam68 antibody: Sam68  binds both cyclin B1 and Erk1/2, but this interaction is inhibited by OA stimulation.	bind
14709	4	5339	6	NULL	NULL	NULL	NULL	OA	Chemical	stimulation of	inhibits					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_1_14_s_186	16221888	(E) Western blot analysis of the IgG, cyclin B1 and Erk1/2  immunoprecipitates from the kinase assay (D) probed with anti-Sam68 antibody: Sam68  binds both cyclin B1 and Erk1/2, but this interaction is inhibited by OA stimulation.	bind
14791	1	5340	5	NULL	NULL	0	NULL	MBP	NULL	bovine	does not bind	NULL				MAG	NULL				NULL		0	NULL	NULL	NULL	gw70_neurobioldis_12_1_1_s_166	12609484	(E) Western blot of bovine MBP after incubation with serum and IgM (data not shown)  bound to several spinal cord proteins, they did not bind to MAG (  Fig. 4B) nor CSPG (  Fig. 4C).	bind
14792	2	5340	5	NULL	NULL	0	NULL	MBP	NULL	bovine	does not bind	NULL				CSPG	NULL				NULL		NULL	NULL	NULL	NULL	gw70_neurobioldis_12_1_1_s_166	12609484	(E) Western blot of bovine MBP after incubation with serum and IgM (data not shown)  bound to several spinal cord proteins, they did not bind to MAG (  Fig. 4B) nor CSPG (  Fig. 4C).	bind
19094	3	5340	5	NULL	NULL	0	NULL	MBP	NULL	bovine	bind	NULL				spinal cord proteins	NULL				NULL		0	NULL	NULL	NULL	gw70_neurobioldis_12_1_1_s_166	12609484	(E) Western blot of bovine MBP after incubation with serum and IgM (data not shown)  bound to several spinal cord proteins, they did not bind to MAG (  Fig. 4B) nor CSPG (  Fig. 4C).	bind
14710	1	5340	6	NULL	NULL	NULL	NULL	MBP	GP	bovine	bind					spinal cord proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_neurobioldis_12_1_1_s_166	12609484	(E) Western blot of bovine MBP after incubation with serum and IgM (data not shown)  bound to several spinal cord proteins, they did not bind to MAG (  Fig. 4B) nor CSPG (  Fig. 4C).	bind
14711	2	5340	6	NULL	NULL	NULL	NULL	MBP	GP	bovine	does not bind					MAG	GP				NULL		NULL	NULL	NULL	NULL	gw70_neurobioldis_12_1_1_s_166	12609484	(E) Western blot of bovine MBP after incubation with serum and IgM (data not shown)  bound to several spinal cord proteins, they did not bind to MAG (  Fig. 4B) nor CSPG (  Fig. 4C).	bind
14712	3	5340	6	NULL	NULL	NULL	NULL	MBP	GP	bovine	does not bind					CSPG	GP				NULL		NULL	NULL	NULL	NULL	gw70_neurobioldis_12_1_1_s_166	12609484	(E) Western blot of bovine MBP after incubation with serum and IgM (data not shown)  bound to several spinal cord proteins, they did not bind to MAG (  Fig. 4B) nor CSPG (  Fig. 4C).	bind
14793	1	5342	5	NULL	NULL	0	NULL	cain	NULL		blocks	NULL				MyHC	NULL	expression of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_17_6600_s_188	10938134	(E) Western blot quantitation revealed a dramatic increase in the amount of total MyHC protein between MyoD and calcineurin, while cain blocked MyHC expression.	bind
14713	1	5342	6	NULL	NULL	NULL	NULL	cain	GP		blocks					MyHC	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6600_s_188	10938134	(E) Western blot quantitation revealed a dramatic increase in the amount of total MyHC protein between MyoD and calcineurin, while cain blocked MyHC expression.	bind
14794	2	5343	5	10	NULL	0	NULL	statement 1			 activate					CRF-R2					NULL		NULL	NULL	NULL	NULL	gw60_neuron_39_3_401_s_115	12895416	(E) When CRF is not bound to CRF-BP, it does not activate CRF-R2.	bind
14795	1	5343	5	10	NULL	0	NULL	CRF			bind					CRF-BP					NULL		NULL	NULL	NULL	NULL	gw60_neuron_39_3_401_s_115	12895416	(E) When CRF is not bound to CRF-BP, it does not activate CRF-R2.	bind
14714	1	5343	6	NULL	NULL	NULL	NULL	CRF	GP		bind					CRF-BP	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_39_3_401_s_115	12895416	(E) When CRF is not bound to CRF-BP, it does not activate CRF-R2.	bind
14715	2	5343	6	NULL	NULL	NULL	NULL	statement 1	Process		activates					CRF-R2	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_39_3_401_s_115	12895416	(E) When CRF is not bound to CRF-BP, it does not activate CRF-R2.	bind
14797	1	5344	5	NULL	NULL	0	NULL	WISH	NULL		bind	NULL		SH3 domain		N-WASP	NULL		proline-rich region		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_3_471_s_87	11157975	(E) WISH SH3 domain binds to the proline-rich region of N-WASP.	bind
14716	1	5344	6	NULL	NULL	NULL	NULL	WISH	GP		bind			SH3 domain		N-WASP	GP		proline-rich region		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_3_471_s_87	11157975	(E) WISH SH3 domain binds to the proline-rich region of N-WASP.	bind
14798	1	5346	5	10	NULL	0	NULL	olfactory receptor neurons		subset of	bind					lectin UEA-1					NULL	P2-Lis1 mice	NULL	NULL	NULL	NULL	gw60_brainres_932_1_1_s_133	11911856	(E, F) The subset of olfactory receptor neurons binding the lectin UEA-1 converge on multiple glomeruli in the ventral region of the olfactory bulb (solid arrows) in both control and P2-Lis1 mice.	bind
14799	4	5346	5	10	NULL	0	NULL	statement 2			converge on					multiple glomeruli		in the ventral region of the olfactory bulb			NULL	in control mice	NULL	NULL	NULL	NULL	gw60_brainres_932_1_1_s_133	11911856	(E, F) The subset of olfactory receptor neurons binding the lectin UEA-1 converge on multiple glomeruli in the ventral region of the olfactory bulb (solid arrows) in both control and P2-Lis1 mice.	bind
14800	3	5346	5	10	NULL	0	NULL	statement 1			converge on					multiple glomeruli		in the ventral region of the olfactory bulb			NULL	in P2-Lis1 mice	NULL	NULL	NULL	NULL	gw60_brainres_932_1_1_s_133	11911856	(E, F) The subset of olfactory receptor neurons binding the lectin UEA-1 converge on multiple glomeruli in the ventral region of the olfactory bulb (solid arrows) in both control and P2-Lis1 mice.	bind
56076	2	5346	5	10	NULL	0	NULL	olfactory receptor neurons			bind					lectin UEA-1					NULL	control mice	0	NULL	NULL	NULL	gw60_brainres_932_1_1_s_133	11911856	(E, F) The subset of olfactory receptor neurons binding the lectin UEA-1 converge on multiple glomeruli in the ventral region of the olfactory bulb (solid arrows) in both control and P2-Lis1 mice.	bind
14717	1	5346	6	NULL	NULL	NULL	NULL	olfactory receptor neurons	OrganismPart		bind					lectin UEA-1	GP				NULL	control mice	NULL	NULL	NULL	NULL	gw60_brainres_932_1_1_s_133	11911856	(E, F) The subset of olfactory receptor neurons binding the lectin UEA-1 converge on multiple glomeruli in the ventral region of the olfactory bulb (solid arrows) in both control and P2-Lis1 mice.	bind
14718	2	5346	6	NULL	NULL	NULL	NULL	olfactory receptor neurons	OrganismPart		bind					lectin UEA-1	GP				NULL	P2-Lis1 mice	NULL	NULL	NULL	NULL	gw60_brainres_932_1_1_s_133	11911856	(E, F) The subset of olfactory receptor neurons binding the lectin UEA-1 converge on multiple glomeruli in the ventral region of the olfactory bulb (solid arrows) in both control and P2-Lis1 mice.	bind
56077	3	5346	6	NULL	NULL	NULL	NULL	statement 1	Process		converge on					multiple glomeruli 	CellComponent	ventral region of the olfactory bulb			NULL	control mice	NULL	NULL	NULL	NULL	gw60_brainres_932_1_1_s_133	11911856	(E, F) The subset of olfactory receptor neurons binding the lectin UEA-1 converge on multiple glomeruli in the ventral region of the olfactory bulb (solid arrows) in both control and P2-Lis1 mice.	bind
56078	4	5346	6	NULL	NULL	NULL	NULL	statement 2	Process		converge on					 multiple glomeruli 	CellComponent	ventral region of the olfactory bulb			NULL	P2-Lis1 mice	NULL	NULL	NULL	NULL	gw60_brainres_932_1_1_s_133	11911856	(E, F) The subset of olfactory receptor neurons binding the lectin UEA-1 converge on multiple glomeruli in the ventral region of the olfactory bulb (solid arrows) in both control and P2-Lis1 mice.	bind
14801	1	5347	5	NULL	NULL	0	NULL	Pin1-/- PGCs	NULL		do not undergo	NULL				apoptosis	NULL	increased			NULL		0	NULL	NULL	NULL	gw60_development_130_15_3579_s_192	12810604	(E,F) Wild-type (E) and  Pin1-mutant (F) PGCs (green, round cells) are not positive for the apoptosis marker LysoTracker (red), indicating that  Pin1-/- PGCs do not undergo increased apoptosis.	bind
14719	1	5347	6	NULL	NULL	NULL	NULL	Pin1-/- PGCs	Cell		do not undergo					apoptosis	Process	increased			NULL		NULL	NULL	NULL	NULL	gw60_development_130_15_3579_s_192	12810604	(E,F) Wild-type (E) and  Pin1-mutant (F) PGCs (green, round cells) are not positive for the apoptosis marker LysoTracker (red), indicating that  Pin1-/- PGCs do not undergo increased apoptosis.	bind
14802	1	5350	5	NULL	NULL	0	NULL	G-CSF	NULL		bind	NULL		E46A		(gp130-Ig)GR	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17445_s_73	10364174	(E46A)G-CSF bound to (gp130-Ig)GR with a similar affinity ( K d = 0.50 nM) to WT G-CSF ( K d = 0.42 nM), indicating that this residue was not required for binding to the CRHM site and probably interacts with the Ig domain.	bind
14803	2	5350	5	NULL	NULL	0	NULL	G-CSF	NULL		bind	NULL		E46A		G-CSF	NULL	WT			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17445_s_73	10364174	(E46A)G-CSF bound to (gp130-Ig)GR with a similar affinity ( K d = 0.50 nM) to WT G-CSF ( K d = 0.42 nM), indicating that this residue was not required for binding to the CRHM site and probably interacts with the Ig domain.	bind
14804	3	5350	5	NULL	NULL	0	NULL	statement 1	NULL		affinity to	NULL	similar			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_25_17445_s_73	10364174	(E46A)G-CSF bound to (gp130-Ig)GR with a similar affinity ( K d = 0.50 nM) to WT G-CSF ( K d = 0.42 nM), indicating that this residue was not required for binding to the CRHM site and probably interacts with the Ig domain.	bind
14805	4	5350	5	NULL	NULL	0	NULL	G-CSF	NULL		is not required for	NULL		E46A			NULL	binding to	CRHM site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17445_s_73	10364174	(E46A)G-CSF bound to (gp130-Ig)GR with a similar affinity ( K d = 0.50 nM) to WT G-CSF ( K d = 0.42 nM), indicating that this residue was not required for binding to the CRHM site and probably interacts with the Ig domain.	bind
14806	5	5350	5	NULL	NULL	0	NULL	G-CSF	NULL		interacts with	NULL	probably	E46A			NULL		Ig domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_25_17445_s_73	10364174	(E46A)G-CSF bound to (gp130-Ig)GR with a similar affinity ( K d = 0.50 nM) to WT G-CSF ( K d = 0.42 nM), indicating that this residue was not required for binding to the CRHM site and probably interacts with the Ig domain.	bind
14720	1	5350	6	NULL	NULL	NULL	NULL	G-CSF	GP		bind			E46A		(gp130-Ig)GR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17445_s_73	10364174	(E46A)G-CSF bound to (gp130-Ig)GR with a similar affinity ( K d = 0.50 nM) to WT G-CSF ( K d = 0.42 nM), indicating that this residue was not required for binding to the CRHM site and probably interacts with the Ig domain.	bind
14721	2	5350	6	NULL	NULL	NULL	NULL	G-CSF	GP		bind			E46A		G-CSF	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17445_s_73	10364174	(E46A)G-CSF bound to (gp130-Ig)GR with a similar affinity ( K d = 0.50 nM) to WT G-CSF ( K d = 0.42 nM), indicating that this residue was not required for binding to the CRHM site and probably interacts with the Ig domain.	bind
14722	3	5350	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs with similar affinity to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17445_s_73	10364174	(E46A)G-CSF bound to (gp130-Ig)GR with a similar affinity ( K d = 0.50 nM) to WT G-CSF ( K d = 0.42 nM), indicating that this residue was not required for binding to the CRHM site and probably interacts with the Ig domain.	bind
14825	4	5350	6	NULL	NULL	NULL	NULL	G-CSF	GP		is not required for			E46A				binding to	CRHM site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17445_s_73	10364174	(E46A)G-CSF bound to (gp130-Ig)GR with a similar affinity ( K d = 0.50 nM) to WT G-CSF ( K d = 0.42 nM), indicating that this residue was not required for binding to the CRHM site and probably interacts with the Ig domain.	bind
14826	5	5350	6	NULL	NULL	NULL	NULL	G-CSF	GP		interacts with		probably	E46A					Ig domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17445_s_73	10364174	(E46A)G-CSF bound to (gp130-Ig)GR with a similar affinity ( K d = 0.50 nM) to WT G-CSF ( K d = 0.42 nM), indicating that this residue was not required for binding to the CRHM site and probably interacts with the Ig domain.	bind
14827	1	5351	5	NULL	NULL	0	NULL	PrPC	NULL		bind	NULL				6H4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_48_38081_s_196	10967124	(Eq. 1)    According to our hypothesis,  A should obey equation 2,           (Eq. 2)    where alpha is a proportionality constant representing the efficiency of PrPC binding to 6H4, of C15S binding to PrPC, of the swine antibody binding to the rabbit antibody, and finally the horseradish peroxidase color reaction.	bind
14828	2	5351	5	NULL	NULL	0	NULL		NULL		bind	NULL		C15S		PrPC	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_48_38081_s_196	10967124	(Eq. 1)    According to our hypothesis,  A should obey equation 2,           (Eq. 2)    where alpha is a proportionality constant representing the efficiency of PrPC binding to 6H4, of C15S binding to PrPC, of the swine antibody binding to the rabbit antibody, and finally the horseradish peroxidase color reaction.	bind
14723	1	5351	6	NULL	NULL	NULL	NULL	PrPC	GP		bind					6H4	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_48_38081_s_196	10967124	(Eq. 1)    According to our hypothesis,  A should obey equation 2,           (Eq. 2)    where alpha is a proportionality constant representing the efficiency of PrPC binding to 6H4, of C15S binding to PrPC, of the swine antibody binding to the rabbit antibody, and finally the horseradish peroxidase color reaction.	bind
14724	2	5351	6	NULL	NULL	NULL	NULL				bind			C15S		PrPC	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_48_38081_s_196	10967124	(Eq. 1)    According to our hypothesis,  A should obey equation 2,           (Eq. 2)    where alpha is a proportionality constant representing the efficiency of PrPC binding to 6H4, of C15S binding to PrPC, of the swine antibody binding to the rabbit antibody, and finally the horseradish peroxidase color reaction.	bind
14829	1	5354	5	NULL	NULL	0	NULL	GALT	NULL	free	does not bind	NULL				UMP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_10_6559_s_210	10037750	(Eq. 1)   But free GALT will not bind UMP to form UMP-GALT ( 34,  35); therefore,  k 5 = 0.	bind
14726	1	5354	6	NULL	NULL	NULL	NULL	GALT	GP	free	does not bind					UMP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_10_6559_s_210	10037750	(Eq. 1)   But free GALT will not bind UMP to form UMP-GALT ( 34,  35); therefore,  k 5 = 0.	bind
14830	1	5355	5	NULL	NULL	0	NULL	Pn	NULL		bind	NULL	irreversibly			AP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_14_13340_s_75	14715654	(Eq. 1) or Pn irreversibly binds to AP and is depleted from the reaction as the PnAP complex as indicated in  Equation 2.	bind
14831	2	5355	5	NULL	NULL	0	NULL	statement 1	NULL		forms	NULL				PnAP complex	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_14_13340_s_75	14715654	(Eq. 1) or Pn irreversibly binds to AP and is depleted from the reaction as the PnAP complex as indicated in  Equation 2.	bind
14727	1	5355	6	NULL	NULL	NULL	NULL	Pn	GP		bind		irreversibly			AP	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_14_13340_s_75	14715654	(Eq. 1) or Pn irreversibly binds to AP and is depleted from the reaction as the PnAP complex as indicated in  Equation 2.	bind
14728	2	5355	6	NULL	NULL	NULL	NULL	statement 1	Process		forms a 					PnAP complex	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_14_13340_s_75	14715654	(Eq. 1) or Pn irreversibly binds to AP and is depleted from the reaction as the PnAP complex as indicated in  Equation 2.	bind
14832	1	5365	5	NULL	NULL	0	NULL	ATP	NULL		bind	NULL				acto-S1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_26974_s_182	15897189	(Eq. 2) and  K1'' k+2'' is the second order rate constant for binding of ATP to acto-S1.	bind
14729	1	5365	6	NULL	NULL	NULL	NULL	ATP	Chemical		bind					acto-S1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_29_26974_s_182	15897189	(Eq. 2) and  K1'' k+2'' is the second order rate constant for binding of ATP to acto-S1.	bind
14833	1	5366	5	NULL	NULL	0	NULL	ATP	NULL		induce	NULL				acto-S1	NULL	dissociation reaction of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_50_50293_s_93	14506231	(Eq. 2) where  kobs represents the observed rate constant for the ATP-induced acto-S1 dissociation reaction,  K1 k+2 is the second order rate constant for the binding of ATP to acto-S1, and  KAD is the equilibrium dissociation constant for ADP binding to acto-S1.	bind
14835	2	5366	5	NULL	NULL	0	NULL	ATP	NULL		bind	NULL				acto-S1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_50_50293_s_93	14506231	(Eq. 2) where  kobs represents the observed rate constant for the ATP-induced acto-S1 dissociation reaction,  K1 k+2 is the second order rate constant for the binding of ATP to acto-S1, and  KAD is the equilibrium dissociation constant for ADP binding to acto-S1.	bind
14837	3	5366	5	NULL	NULL	0	NULL	ADP	NULL		bind	NULL				acto-S1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_50_50293_s_93	14506231	(Eq. 2) where  kobs represents the observed rate constant for the ATP-induced acto-S1 dissociation reaction,  K1 k+2 is the second order rate constant for the binding of ATP to acto-S1, and  KAD is the equilibrium dissociation constant for ADP binding to acto-S1.	bind
14730	1	5366	6	NULL	NULL	NULL	NULL	ATP	Chemical		bind					acto-S1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_50_50293_s_93	14506231	(Eq. 2) where  kobs represents the observed rate constant for the ATP-induced acto-S1 dissociation reaction,  K1 k+2 is the second order rate constant for the binding of ATP to acto-S1, and  KAD is the equilibrium dissociation constant for ADP binding to acto-S1.	bind
14731	2	5366	6	NULL	NULL	NULL	NULL	ADP	Chemical		bind					acto-S1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_50_50293_s_93	14506231	(Eq. 2) where  kobs represents the observed rate constant for the ATP-induced acto-S1 dissociation reaction,  K1 k+2 is the second order rate constant for the binding of ATP to acto-S1, and  KAD is the equilibrium dissociation constant for ADP binding to acto-S1.	bind
56079	3	5366	6	NULL	NULL	NULL	NULL	ATP	Chemical		induce					acto-S1 	GP	dissociation reaction of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_50_50293_s_93	14506231	(Eq. 2) where  kobs represents the observed rate constant for the ATP-induced acto-S1 dissociation reaction,  K1 k+2 is the second order rate constant for the binding of ATP to acto-S1, and  KAD is the equilibrium dissociation constant for ADP binding to acto-S1.	bind
15606	1	5367	5	NULL	NULL	0	NULL	CheA	NULL		bind	NULL				CF	NULL	WT			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_41_30512_s_72	16920717	(Eq. 2) where Act o and Act* are the CheA activities bound to 100% WT-CF and 100% NS-CF arrays, respectively; and [ CoA] and [ C*A are the CheA concentrations bound to WT- and NS-CFs, respectively (in the presence of CheW), estimated through the model with constraints imposed by the activity and binding data.	bind
15607	2	5367	5	NULL	NULL	0	NULL	statement 1	NULL		in the presence of	NULL				CheW	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_41_30512_s_72	16920717	(Eq. 2) where Act o and Act* are the CheA activities bound to 100% WT-CF and 100% NS-CF arrays, respectively; and [ CoA] and [ C*A are the CheA concentrations bound to WT- and NS-CFs, respectively (in the presence of CheW), estimated through the model with constraints imposed by the activity and binding data.	bind
15608	3	5367	5	NULL	NULL	0	NULL	CheA	NULL		bind	NULL				CF	NULL	NS			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_41_30512_s_72	16920717	(Eq. 2) where Act o and Act* are the CheA activities bound to 100% WT-CF and 100% NS-CF arrays, respectively; and [ CoA] and [ C*A are the CheA concentrations bound to WT- and NS-CFs, respectively (in the presence of CheW), estimated through the model with constraints imposed by the activity and binding data.	bind
19163	4	5367	5	NULL	NULL	0	NULL	statement 3	NULL		in the presence of	NULL				CheW	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_41_30512_s_72	16920717	(Eq. 2) where Act o and Act* are the CheA activities bound to 100% WT-CF and 100% NS-CF arrays, respectively; and [ CoA] and [ C*A are the CheA concentrations bound to WT- and NS-CFs, respectively (in the presence of CheW), estimated through the model with constraints imposed by the activity and binding data.	bind
19028	1	5367	6	NULL	NULL	NULL	NULL	CheA	GP		bind					CF	GP	NS			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_41_30512_s_72	16920717	(Eq. 2) where Act o and Act* are the CheA activities bound to 100% WT-CF and 100% NS-CF arrays, respectively; and [ CoA] and [ C*A are the CheA concentrations bound to WT- and NS-CFs, respectively (in the presence of CheW), estimated through the model with constraints imposed by the activity and binding data.	bind
19029	2	5367	6	NULL	NULL	NULL	NULL	CheA	GP		bind					CF	GP	WT			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_41_30512_s_72	16920717	(Eq. 2) where Act o and Act* are the CheA activities bound to 100% WT-CF and 100% NS-CF arrays, respectively; and [ CoA] and [ C*A are the CheA concentrations bound to WT- and NS-CFs, respectively (in the presence of CheW), estimated through the model with constraints imposed by the activity and binding data.	bind
19816	3	5367	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs in presence of					CheW	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_41_30512_s_72	16920717	(Eq. 2) where Act o and Act* are the CheA activities bound to 100% WT-CF and 100% NS-CF arrays, respectively; and [ CoA] and [ C*A are the CheA concentrations bound to WT- and NS-CFs, respectively (in the presence of CheW), estimated through the model with constraints imposed by the activity and binding data.	bind
19817	4	5367	6	NULL	NULL	NULL	NULL	statement 2	Process		occurs in presence of					CheW	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_41_30512_s_72	16920717	(Eq. 2) where Act o and Act* are the CheA activities bound to 100% WT-CF and 100% NS-CF arrays, respectively; and [ CoA] and [ C*A are the CheA concentrations bound to WT- and NS-CFs, respectively (in the presence of CheW), estimated through the model with constraints imposed by the activity and binding data.	bind
14840	1	5369	5	NULL	NULL	0	NULL	ARNT-bHLH dimers	NULL		bind	NULL				ARNT-bHLH dimer	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_44_40537_s_125	11502749	(Eq. 3)    where nu2 is the average number of ARNT-bHLH dimers bound to the ARNT-bHLH dimer.	bind
14841	2	5369	5	NULL	NULL	0	NULL	nu2	NULL		is	NULL				average number of ARNT-bHLH dimers bound to the ARNT-bHLH dimer	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_44_40537_s_125	11502749	(Eq. 3)    where nu2 is the average number of ARNT-bHLH dimers bound to the ARNT-bHLH dimer.	bind
14732	1	5369	6	NULL	NULL	NULL	NULL	ARNT-bHLH dimers	GP		bind					ARNT-bHLH dimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_40537_s_125	11502749	(Eq. 3)    where nu2 is the average number of ARNT-bHLH dimers bound to the ARNT-bHLH dimer.	bind
56080	2	5369	6	NULL	NULL	NULL	NULL	nu2	GP		is					average number of ARNT-bHLH dimers bound to the ARNT-bHLH dimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_40537_s_125	11502749	(Eq. 3)    where nu2 is the average number of ARNT-bHLH dimers bound to the ARNT-bHLH dimer.	bind
14843	1	5370	5	10	NULL	0	NULL	 IdeR		active	bind					fxbA				operator region	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_51_53554_s_146	15456786	(Eq. 3)  Kd is the equilibrium dissociation constant where half of the IdeR is activated and bound to the  fxbA operator region,  M is the divalent metal ion concentration, and  h is the Hill coefficient, which is often used as a measurement of cooperativity.	bind
14733	1	5370	6	NULL	NULL	NULL	NULL	IdeR	GP	activated	bind					fxbA	GP			operator	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_51_53554_s_146	15456786	(Eq. 3)  Kd is the equilibrium dissociation constant where half of the IdeR is activated and bound to the  fxbA operator region,  M is the divalent metal ion concentration, and  h is the Hill coefficient, which is often used as a measurement of cooperativity.	bind
14844	1	5371	5	NULL	NULL	0	NULL	pAB	NULL		bind	NULL				FXa subforms	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_28_16621_s_63	8663222	(Eq. 3)  pAB Binding to FXa Subforms	bind
14734	1	5371	6	NULL	NULL	NULL	NULL	pAB	GP		bind					FXa subforms	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_28_16621_s_63	8663222	(Eq. 3)  pAB Binding to FXa Subforms	bind
14845	1	5372	5	NULL	NULL	0	NULL	i CytR dimers	NULL		bind	NULL				udp	NULL	unliganded 		promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_23_16010_s_149	10347150	(Eq. 3) delta G i,M is the free energy change for binding of  i CytR dimers to the unliganded  udp promoter ( i.e. related to the macroscopic product association equilibrium constant by  K i,M =          The value of  N in   N was treated as an adjustable parameter in the analysis, representing the average CytR stoichiometry of the higher order complexes.	bind
14735	1	5372	6	NULL	NULL	NULL	NULL	i CytR dimers	GP		bind					udp	GP	unliganded		promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_23_16010_s_149	10347150	(Eq. 3) delta G i,M is the free energy change for binding of  i CytR dimers to the unliganded  udp promoter ( i.e. related to the macroscopic product association equilibrium constant by  K i,M =          The value of  N in   N was treated as an adjustable parameter in the analysis, representing the average CytR stoichiometry of the higher order complexes.	bind
14847	1	5373	5	NULL	NULL	0	NULL	GCLC	NULL		bind	NULL				GCLM	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_40_33766_s_133	16081425	(Eq. 3) The total GCL activity (GCLtot) when all GCLC is bound with GCLM is as follows.	bind
14736	1	5373	6	NULL	NULL	NULL	NULL	GCLC	GP		bind					GCLM	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_40_33766_s_133	16081425	(Eq. 3) The total GCL activity (GCLtot) when all GCLC is bound with GCLM is as follows.	bind
15604	1	5379	5	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				Gi	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_2_922_s_92	11689554	(Eq. 5)    The dissociation constant for GTP binding to Gi ( K i) was determined from the inhibition of the initial rate of GTPgammaS binding (Equation  6), where I is GTP,  K s is the Michaelis constant for GTPgammaS, and  V is the maximum velocity.	bind
14737	1	5379	6	NULL	NULL	NULL	NULL	GTP	Chemical		bind					Gi					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_2_922_s_92	11689554	(Eq. 5)    The dissociation constant for GTP binding to Gi ( K i) was determined from the inhibition of the initial rate of GTPgammaS binding (Equation  6), where I is GTP,  K s is the Michaelis constant for GTPgammaS, and  V is the maximum velocity.	bind
14849	1	5380	5	NULL	NULL	0	NULL	PRPP	NULL		bind	NULL				UMP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_9_6921_s_177	12482852	(Eq. 5)    We consider this agreement to be acceptable given that the value for the Michaelis  constant for PPi could not be determined very accurately and that the dissociation constants for binding of PRPP and UMP used for estimates of the corresponding inhibition constants were determined at pH 7.5 and 0  degrees C.	bind
19032	1	5380	6	NULL	NULL	NULL	NULL	PRPP	GP		bind					UMP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_9_6921_s_177	12482852	(Eq. 5)    We consider this agreement to be acceptable given that the value for the Michaelis  constant for PPi could not be determined very accurately and that the dissociation constants for binding of PRPP and UMP used for estimates of the corresponding inhibition constants were determined at pH 7.5 and 0  degrees C.	bind
14850	1	5382	5	10	NULL	0	NULL	ADP			bind					GSTKar3 complex		Mt			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_49_51354_s_135	15385545	(Eq. 5) where Mt.E.ADP is the concentration of ADP bound to Mt.GSTKar3 complex,  E0 is the total GSTKar3 concentration, ADP is the total nucleotide present, and  Kd is the dissociation constant for ADP.	bind
14738	1	5382	6	NULL	NULL	NULL	NULL	ADP	Chemical		bind					GSTKar3 complex	GP	Mt			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_49_51354_s_135	15385545	(Eq. 5) where Mt.E.ADP is the concentration of ADP bound to Mt.GSTKar3 complex,  E0 is the total GSTKar3 concentration, ADP is the total nucleotide present, and  Kd is the dissociation constant for ADP.	bind
14853	1	5383	5	NULL	NULL	0	NULL	Rb+	NULL		bind	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_8_5922_s_77	11739378	(Eq. 6)    quation  6 contains all the terms predicted by the stoichiometry of binding of Rb+ and ATP, which suggests that all the possible states of the enzyme with bound ATP and/or bound or occluded Rb+ are present in equilibrium with free Rb+ and ATP.	bind
14739	1	5383	6	NULL	NULL	NULL	NULL	Rb+	Chemical		bind					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_8_5922_s_77	11739378	(Eq. 6)    quation  6 contains all the terms predicted by the stoichiometry of binding of Rb+ and ATP, which suggests that all the possible states of the enzyme with bound ATP and/or bound or occluded Rb+ are present in equilibrium with free Rb+ and ATP.	bind
14868	1	5385	5	NULL	NULL	0	NULL	hirudin	NULL		bind	NULL				thrombin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_26997_s_60	15923186	(Eq. 7) where  k1 is the second-order rate constant for hirudin binding to thrombin.	bind
14742	1	5385	6	NULL	NULL	NULL	NULL	hirudin	GP		bind					thrombin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_29_26997_s_60	15923186	(Eq. 7) where  k1 is the second-order rate constant for hirudin binding to thrombin.	bind
14870	1	5387	5	NULL	NULL	0	NULL	GST-HuR	NULL		bind	NULL				RNA substrates	NULL	Fl-labeled 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_23_22406_s_110	15809297	(Eq. 9) Quantitative assessment of binding between GST-HuR and Fl-labeled RNA substrates was similarly preformed using fluorescence anisotropy, but with two significant variations.	bind
14743	1	5387	6	NULL	NULL	NULL	NULL	GST-HuR	GP		bind					RNA	NucleicAcid	F1-labeled			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_23_22406_s_110	15809297	(Eq. 9) Quantitative assessment of binding between GST-HuR and Fl-labeled RNA substrates was similarly preformed using fluorescence anisotropy, but with two significant variations.	bind
14871	1	5388	5	NULL	NULL	0	NULL	PMCA	NULL		bind	NULL				calmodulin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_43_39797_s_296	11514555	(Eq. A1)[[             ]](Eq. A2)    The concentration of PMCA bound to calmodulin, [PC], can be expressed in terms of [PCCa] and [P] by using the following mass conservation equation.	bind
14744	1	5388	6	NULL	NULL	NULL	NULL	PMCA	GP		bind					calmodulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_43_39797_s_296	11514555	(Eq. A1)[[             ]](Eq. A2)    The concentration of PMCA bound to calmodulin, [PC], can be expressed in terms of [PCCa] and [P] by using the following mass conservation equation.	bind
14745	1	5389	6	NULL	NULL	NULL	NULL	phosphoprotein 50	GP		bind					ERM	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_6_2372_s_159	12808036	(ERM-binding phosphoprotein 50) and a number of  membrane proteins and a C-terminal domain (C-ERMAD) harboring the F-actin  binding site (for reviews see Bretscher  et al.,  2000  ,  2002  ;  Tsukita  et al., 1997  ;  Mangeat  et al.,  1999  ).	bind
14872	1	5390	5	NULL	NULL	0	NULL	ER 	NULL		bind	NULL				alpha2 integrin	NULL		I domain		NULL		0	NULL	NULL	NULL	gw70_cellbiol_166_1_97_s_126	15240572	(F and G) Analyses of ER and LG3 binding to the I domain  of alpha2 integrin by SPR.	bind
14873	2	5390	5	NULL	NULL	0	NULL	LG3	NULL		bind	NULL				alpha2 integrin	NULL		I domain		NULL		0	NULL	NULL	NULL	gw70_cellbiol_166_1_97_s_126	15240572	(F and G) Analyses of ER and LG3 binding to the I domain  of alpha2 integrin by SPR.	bind
14746	1	5390	6	NULL	NULL	NULL	NULL	ER	CellComponent		bind					alpha2 integrin	GP		I domain		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_166_1_97_s_126	15240572	(F and G) Analyses of ER and LG3 binding to the I domain  of alpha2 integrin by SPR.	bind
14747	2	5390	6	NULL	NULL	NULL	NULL	LG3	GP		bind					alpha2 integrin	GP		I domain		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_166_1_97_s_126	15240572	(F and G) Analyses of ER and LG3 binding to the I domain  of alpha2 integrin by SPR.	bind
14874	1	5391	5	NULL	NULL	0	NULL	Smad7	NULL		bind	NULL				GADD34	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_164_2_291_s_47	14718519	(f and g) Similar experiments were performed in both yeast  (f) and mammalian (g) systems to map Smad7 binding to GADD34.	bind
14748	1	5391	6	NULL	NULL	NULL	NULL	Smad7	GP		bind					GADD34	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_291_s_47	14718519	(f and g) Similar experiments were performed in both yeast  (f) and mammalian (g) systems to map Smad7 binding to GADD34.	bind
14875	1	5392	5	10	NULL	0	NULL	neurofilament fragments	NULL	sonicated	bind	NULL				microtubules	NULL	along the side of			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_11_5092_s_136	15342782	(f and g) Sonicated neurofilament fragments bind along the  side of microtubules in the presence of dynein/dynactin In the absence of dynein/dynactin  less binding of sonicated NF fragments to microtubules is seen (our unpublished results).	bind
14876	2	5392	5	NULL	NULL	0	NULL	statement 1	NULL		in the presence of	NULL				dynein/dynactin	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_11_5092_s_136	15342782	(f and g) Sonicated neurofilament fragments bind along the  side of microtubules in the presence of dynein/dynactin In the absence of dynein/dynactin  less binding of sonicated NF fragments to microtubules is seen (our unpublished results).	bind
14877	3	5392	5	NULL	NULL	0	NULL	NF fragments	NULL	sonicated	bind	NULL	lesser			microtubules	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_11_5092_s_136	15342782	(f and g) Sonicated neurofilament fragments bind along the  side of microtubules in the presence of dynein/dynactin In the absence of dynein/dynactin  less binding of sonicated NF fragments to microtubules is seen (our unpublished results).	bind
14878	4	5392	5	NULL	NULL	0	NULL	statement 3	NULL		in the absence of	NULL				dynein/dynactin	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_11_5092_s_136	15342782	(f and g) Sonicated neurofilament fragments bind along the  side of microtubules in the presence of dynein/dynactin In the absence of dynein/dynactin  less binding of sonicated NF fragments to microtubules is seen (our unpublished results).	bind
14749	1	5392	6	NULL	NULL	NULL	NULL	neurofilament fragments	CellComponent	sonicated	bind					 microtubules 	CellComponent	side of			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_11_5092_s_136	15342782	(f and g) Sonicated neurofilament fragments bind along the  side of microtubules in the presence of dynein/dynactin In the absence of dynein/dynactin  less binding of sonicated NF fragments to microtubules is seen (our unpublished results).	bind
19033	2	5392	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs in presence of					dynein/dynactin	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_11_5092_s_136	15342782	(f and g) Sonicated neurofilament fragments bind along the  side of microtubules in the presence of dynein/dynactin In the absence of dynein/dynactin  less binding of sonicated NF fragments to microtubules is seen (our unpublished results).	bind
19034	3	5392	6	NULL	NULL	NULL	NULL	NF fragments	CellComponent	sonicated	bind		less			microtubules	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_11_5092_s_136	15342782	(f and g) Sonicated neurofilament fragments bind along the  side of microtubules in the presence of dynein/dynactin In the absence of dynein/dynactin  less binding of sonicated NF fragments to microtubules is seen (our unpublished results).	bind
19035	4	5392	6	NULL	NULL	NULL	NULL	statement 3	Process		occurs in absence of					dynein/dynactin	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_11_5092_s_136	15342782	(f and g) Sonicated neurofilament fragments bind along the  side of microtubules in the presence of dynein/dynactin In the absence of dynein/dynactin  less binding of sonicated NF fragments to microtubules is seen (our unpublished results).	bind
14879	1	5393	5	10	NULL	0	NULL	(F Pmp) -TAM			bind					ZAP-70			tandem SH2 domains		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_944_s_69	7822334	(F Pmp) -TAM    bound the tandem  SH2 domains of ZAP-70 with an affinity similar to the  (pTyr) -TAM    itself.	bind
14880	2	5393	5	10	NULL	0	NULL	TAM			bind			pTyr		ZAP-70			tandem SH2 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_944_s_69	7822334	(F Pmp) -TAM    bound the tandem  SH2 domains of ZAP-70 with an affinity similar to the  (pTyr) -TAM    itself.	bind
14881	3	5393	5	10	NULL	0	NULL	statement 1			is similar to					statement 2					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_944_s_69	7822334	(F Pmp) -TAM    bound the tandem  SH2 domains of ZAP-70 with an affinity similar to the  (pTyr) -TAM    itself.	bind
14750	1	5393	6	NULL	NULL	NULL	NULL	(F Pmp) -TAM	GP		bind					ZAP-70	GP		tandem SH2 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_944_s_69	7822334	(F Pmp) -TAM    bound the tandem  SH2 domains of ZAP-70 with an affinity similar to the  (pTyr) -TAM    itself.	bind
19036	2	5393	6	NULL	NULL	NULL	NULL	TAM	GP		bind			pTyr		ZAP-70	GP		tandem SH2 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_944_s_69	7822334	(F Pmp) -TAM    bound the tandem  SH2 domains of ZAP-70 with an affinity similar to the  (pTyr) -TAM    itself.	bind
19037	3	5393	6	NULL	NULL	NULL	NULL	statement 1	Process		is similar to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_944_s_69	7822334	(F Pmp) -TAM    bound the tandem  SH2 domains of ZAP-70 with an affinity similar to the  (pTyr) -TAM    itself.	bind
14882	1	5394	5	NULL	NULL	0	NULL	CNP	NULL		bind	NULL				tubulin	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_170_4_661_s_75	16103231	(F)  Comparison of CNP and tau binding to tubulin.	bind
14883	2	5394	5	NULL	NULL	0	NULL	tau	NULL		bind	NULL				tubulin	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_170_4_661_s_75	16103231	(F)  Comparison of CNP and tau binding to tubulin.	bind
14751	1	5394	6	NULL	NULL	NULL	NULL	CNP	GP		bind					tubulin	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_170_4_661_s_75	16103231	(F)  Comparison of CNP and tau binding to tubulin.	bind
14755	2	5394	6	NULL	NULL	NULL	NULL	tau	GP		bind					tubulin	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_170_4_661_s_75	16103231	(F)  Comparison of CNP and tau binding to tubulin.	bind
14884	1	5395	5	NULL	NULL	0	NULL	InR	NULL		bind	NULL				GST-IRS	NULL	WT	1108 - 516		NULL		0	NULL	NULL	NULL	gw70_cellbiol_166_2_213_s_181	15249583	(F)  Quantitation of InR binding to GST-IRS-1108 - 516 (WT) or S302A and S302E mutants.	bind
14885	2	5395	5	NULL	NULL	0	NULL	InR	NULL		bind	NULL				GST-IRS	NULL	mutant	S302A		NULL		0	NULL	NULL	NULL	gw70_cellbiol_166_2_213_s_181	15249583	(F)  Quantitation of InR binding to GST-IRS-1108 - 516 (WT) or S302A and S302E mutants.	bind
14886	3	5395	5	NULL	NULL	0	NULL	InR	NULL		bind	NULL				GST-IRS	NULL	mutant	S302E		NULL		0	NULL	NULL	NULL	gw70_cellbiol_166_2_213_s_181	15249583	(F)  Quantitation of InR binding to GST-IRS-1108 - 516 (WT) or S302A and S302E mutants.	bind
14761	1	5395	6	NULL	NULL	NULL	NULL	InR	GP		bind					GST-IRS	GP	wild type	1108 - 516		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_166_2_213_s_181	15249583	(F)  Quantitation of InR binding to GST-IRS-1108 - 516 (WT) or S302A and S302E mutants.	bind
14762	2	5395	6	NULL	NULL	NULL	NULL	InR	GP		bind					GST-IRS	GP	mutant	S302A		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_166_2_213_s_181	15249583	(F)  Quantitation of InR binding to GST-IRS-1108 - 516 (WT) or S302A and S302E mutants.	bind
14765	3	5395	6	NULL	NULL	NULL	NULL	InR	GP		bind					GST-IRS	GP	mutant	S302E		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_166_2_213_s_181	15249583	(F)  Quantitation of InR binding to GST-IRS-1108 - 516 (WT) or S302A and S302E mutants.	bind
14887	1	5396	5	NULL	NULL	0	NULL	PMP	NULL	cytosolic	bind	NULL				PEX19	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_164_1_57_s_53	14709540	(F)  The majority of cytosolic PMP is bound to PEX19.	bind
14768	1	5396	6	NULL	NULL	NULL	NULL	PMP	GP	cytosolic	bind					PEX19	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_1_57_s_53	14709540	(F)  The majority of cytosolic PMP is bound to PEX19.	bind
14888	1	5397	5	NULL	NULL	0	NULL	ERK2	NULL		bind	NULL				Mxi2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_9_3079_s_225	12697810	(F) Affinity of ERK2 binding to Mxi2.	bind
14770	1	5397	6	NULL	NULL	NULL	NULL	ERK2	GP		bind					Mxi2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_9_3079_s_225	12697810	(F) Affinity of ERK2 binding to Mxi2.	bind
14889	1	5398	5	10	NULL	0	NULL	Robo1/Fc			bind					Slit2-expressing cells					NULL		NULL	NULL	NULL	NULL	gw70_devbiol_296_2_499_s_544	16854408	(F) Anti-Fc labeling reveals that Robo1/Fc successfully binds  to Slit2-expressing cells, but not  Mock  cells (data not shown) in a collagen gel.	bind
14890	2	5398	5	10	NULL	0	NULL	Robo1/Fc			does not bind					Mock cells 					NULL		NULL	NULL	NULL	NULL	gw70_devbiol_296_2_499_s_544	16854408	(F) Anti-Fc labeling reveals that Robo1/Fc successfully binds  to Slit2-expressing cells, but not  Mock  cells (data not shown) in a collagen gel.	bind
14807	1	5398	6	NULL	NULL	NULL	NULL	Robo1/Fc	GP		bind					Slit2-expressing cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_296_2_499_s_544	16854408	(F) Anti-Fc labeling reveals that Robo1/Fc successfully binds  to Slit2-expressing cells, but not  Mock  cells (data not shown) in a collagen gel.	bind
14808	2	5398	6	NULL	NULL	NULL	NULL	Robo1/Fc	GP		does not bind					Mock cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_296_2_499_s_544	16854408	(F) Anti-Fc labeling reveals that Robo1/Fc successfully binds  to Slit2-expressing cells, but not  Mock  cells (data not shown) in a collagen gel.	bind
14891	1	5399	5	NULL	NULL	0	NULL	EF-G-GTP	NULL		bind	NULL				ribosome	NULL	pre-translocational state of			NULL		0	NULL	NULL	NULL	gw60_structure_4_3_229_s_280	8805530	(f) Binding of EF-G-GTP to the pre-translocational state of the ribosome.	bind
14809	1	5399	6	NULL	NULL	NULL	NULL	EF-G-GTP	Chemical		bind					ribosome	CellComponent	pre-translocational state of			NULL		NULL	NULL	NULL	NULL	gw60_structure_4_3_229_s_280	8805530	(f) Binding of EF-G-GTP to the pre-translocational state of the ribosome.	bind
14892	1	5400	5	10	NULL	NULL	NULL	Hrs	GP		bind					STAM2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_9_3675_s_87	12972556	(F) Binding of Hrs to STAM2 and its mutants.	bind
14893	2	5400	5	10	NULL	NULL	NULL	Hrs	GP		bind					STAM2	GP	mutants			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_9_3675_s_87	12972556	(F) Binding of Hrs to STAM2 and its mutants.	bind
14810	1	5400	6	10	NULL	NULL	NULL	Hrs	GP		bind					STAM2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_9_3675_s_87	12972556	(F) Binding of Hrs to STAM2 and its mutants.	bind
14811	2	5400	6	10	NULL	NULL	NULL	Hrs	GP		bind					STAM2	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_9_3675_s_87	12972556	(F) Binding of Hrs to STAM2 and its mutants.	bind
14954	1	5401	6	10	NULL	NULL	NULL	Pax1	GP		bind					oligonucleotide S1	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_130_3_473_s_135	12490554	(F) Binding of Pax1 and Pax9 to oligonucleotide  S1.	bind
14955	2	5401	6	10	NULL	NULL	NULL	Pax9	GP		bind					oligonucleotide S1	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_130_3_473_s_135	12490554	(F) Binding of Pax1 and Pax9 to oligonucleotide  S1.	bind
15277	1	5401	7	10	NULL	NULL	NULL	Pax1	GP		bind					 oligonucleotide S1	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_130_3_473_s_135	12490554	(F) Binding of Pax1 and Pax9 to oligonucleotide  S1.	bind
15278	2	5401	7	10	NULL	NULL	NULL	Pax9	GP		bind					oligonucleotide S1	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_130_3_473_s_135	12490554	(F) Binding of Pax1 and Pax9 to oligonucleotide  S1.	bind
14956	1	5403	6	10	NULL	NULL	NULL	TBP	GP		bind					GAL1 	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_18_6270_s_220	11509669	(F) Binding of TBP to the  GAL1 and  GAL10 promoters.	bind
14957	2	5403	6	10	NULL	NULL	NULL	TBP	GP		bind					GAL10	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_18_6270_s_220	11509669	(F) Binding of TBP to the  GAL1 and  GAL10 promoters.	bind
15284	1	5403	7	10	NULL	NULL	NULL	TBP	GP		bind					GAL1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_18_6270_s_220	11509669	(F) Binding of TBP to the  GAL1 and  GAL10 promoters.	bind
15285	2	5403	7	10	NULL	NULL	NULL	TBP	GP		bind					GAL10	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_18_6270_s_220	11509669	(F) Binding of TBP to the  GAL1 and  GAL10 promoters.	bind
14961	1	5404	6	10	NULL	NULL	NULL	SBP	GP		bind					sperm LD-DIM	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_43_42050_s_101	12917406	(f) Binding of the SBP to the Sperm LD-DIM and the Sialidase-treated One --	bind
15286	1	5404	7	10	NULL	NULL	NULL	SBP	GP		bind					Sperm LD-DIM	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_43_42050_s_101	12917406	(f) Binding of the SBP to the Sperm LD-DIM and the Sialidase-treated One --	bind
14962	1	5405	6	10	NULL	NULL	NULL	Sed5	GP		bind			LxxME		Sec24	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_4_483_s_234	12941276	(F) Binding of the Sed5 LxxME sequence to Sec24 is not affected by the assembly state.	bind
19038	2	5405	6	10	NULL	NULL	NULL	statement 1	Process		is not affected by					assembly state	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_4_483_s_234	12941276	(F) Binding of the Sed5 LxxME sequence to Sec24 is not affected by the assembly state.	bind
15287	1	5405	7	10	NULL	NULL	NULL	Sed5 	GP		bind			LxxME sequence		Sec24	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_4_483_s_234	12941276	(F) Binding of the Sed5 LxxME sequence to Sec24 is not affected by the assembly state.	bind
15288	2	5405	7	10	NULL	NULL	NULL	statement 1	Process		is not affected by					assembly state	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_4_483_s_234	12941276	(F) Binding of the Sed5 LxxME sequence to Sec24 is not affected by the assembly state.	bind
14963	1	5406	6	10	NULL	NULL	NULL	syntaxin-1A	GP		bind					myosin-V	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_212	16030255	(F) Ca2+ requirement for binding of syntaxin-1A to myosin-V is due to Ca2+-dependent release of CaM from the neck domain of myosin-Va.	bind
14964	2	5406	6	10	NULL	NULL	NULL	statement 1	Process		requires					Ca+2	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_212	16030255	(F) Ca2+ requirement for binding of syntaxin-1A to myosin-V is due to Ca2+-dependent release of CaM from the neck domain of myosin-Va.	bind
14966	3	5406	6	10	NULL	NULL	NULL	myosin-Va	GP		release			neck domain		CaM	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_212	16030255	(F) Ca2+ requirement for binding of syntaxin-1A to myosin-V is due to Ca2+-dependent release of CaM from the neck domain of myosin-Va.	bind
14967	4	5406	6	10	NULL	NULL	NULL	statement 3	Process		is dependent on					Ca+2	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_212	16030255	(F) Ca2+ requirement for binding of syntaxin-1A to myosin-V is due to Ca2+-dependent release of CaM from the neck domain of myosin-Va.	bind
14968	5	5406	6	10	NULL	NULL	NULL	statement 2	Process		is due to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_212	16030255	(F) Ca2+ requirement for binding of syntaxin-1A to myosin-V is due to Ca2+-dependent release of CaM from the neck domain of myosin-Va.	bind
15291	1	5406	7	10	NULL	NULL	NULL	syntaxin-1A 	GP		bind					myosin-V	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_212	16030255	(F) Ca2+ requirement for binding of syntaxin-1A to myosin-V is due to Ca2+-dependent release of CaM from the neck domain of myosin-Va.	bind
15292	2	5406	7	10	NULL	NULL	NULL	statement 1	Process		is dependent on					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_212	16030255	(F) Ca2+ requirement for binding of syntaxin-1A to myosin-V is due to Ca2+-dependent release of CaM from the neck domain of myosin-Va.	bind
15293	3	5406	7	10	NULL	NULL	NULL	myosin-Va	GP		release			neck domain		CaM	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_212	16030255	(F) Ca2+ requirement for binding of syntaxin-1A to myosin-V is due to Ca2+-dependent release of CaM from the neck domain of myosin-Va.	bind
15294	5	5406	7	10	NULL	NULL	NULL	statement 2	Process		is due to 					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_212	16030255	(F) Ca2+ requirement for binding of syntaxin-1A to myosin-V is due to Ca2+-dependent release of CaM from the neck domain of myosin-Va.	bind
44716	4	5406	7	10	NULL	NULL	NULL	statement 3	Process		is dependent on					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_212	16030255	(F) Ca2+ requirement for binding of syntaxin-1A to myosin-V is due to Ca2+-dependent release of CaM from the neck domain of myosin-Va.	bind
14971	1	5407	6	10	NULL	NULL	NULL	CCD vesicles	CellComponent		bind		specifically			COG complex	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_cellbiol_168_5_747_s_114	15728195	(F) CCD vesicles  specifically bind to the COG complex in vitro.	bind
15295	1	5407	7	10	NULL	NULL	NULL	CCD vesicles	CellComponent		bind		specifically			COG complex	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_cellbiol_168_5_747_s_114	15728195	(F) CCD vesicles  specifically bind to the COG complex in vitro.	bind
14974	1	5408	6	10	NULL	NULL	NULL	INCENP	GP	chicken	bind					AIRK2	GP	human			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_currbiol_10_17_1075_s_27	10996078	(f) Chicken INCENP (cINCENP) binds human AIRK2  in vitro.	bind
19039	2	5408	6	10	NULL	NULL	NULL	Chicken INCENP	GP		is					cINCENP	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_17_1075_s_27	10996078	(f) Chicken INCENP (cINCENP) binds human AIRK2  in vitro.	bind
15296	1	5408	7	10	NULL	NULL	NULL	INCENP	GP	chicken	bind					AIRK2	GP	human			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_currbiol_10_17_1075_s_27	10996078	(f) Chicken INCENP (cINCENP) binds human AIRK2  in vitro.	bind
15297	2	5408	7	10	NULL	NULL	NULL	Chicken INCENP	GP		is					cINCENP	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_17_1075_s_27	10996078	(f) Chicken INCENP (cINCENP) binds human AIRK2  in vitro.	bind
14977	1	5409	6	10	NULL	NULL	NULL	Myc	GP		bind					p21 initiator	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcell_10_3_509_s_201	12408820	(F) Chromatin-immunoprecipitation assay (ChIP) documenting binding of Myc and Miz-1 to the p21 initiator in vivo; control panels show ChIP reactions for the E box of the prothymosin-  gene and the coding region of the p15Ink4b gene as negative control  (Staller et al., 2001  ).	bind
14978	2	5409	6	10	NULL	NULL	NULL	Miz-1	GP		bind					p21 initiator	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcell_10_3_509_s_201	12408820	(F) Chromatin-immunoprecipitation assay (ChIP) documenting binding of Myc and Miz-1 to the p21 initiator in vivo; control panels show ChIP reactions for the E box of the prothymosin-  gene and the coding region of the p15Ink4b gene as negative control  (Staller et al., 2001  ).	bind
15298	1	5409	7	10	NULL	NULL	NULL	Myc	GP		bind					p21 initiator	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcell_10_3_509_s_201	12408820	(F) Chromatin-immunoprecipitation assay (ChIP) documenting binding of Myc and Miz-1 to the p21 initiator in vivo; control panels show ChIP reactions for the E box of the prothymosin-  gene and the coding region of the p15Ink4b gene as negative control  (Staller et al., 2001  ).	bind
15299	2	5409	7	10	NULL	NULL	NULL	Miz-1	GP		bind					p21 initiator	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcell_10_3_509_s_201	12408820	(F) Chromatin-immunoprecipitation assay (ChIP) documenting binding of Myc and Miz-1 to the p21 initiator in vivo; control panels show ChIP reactions for the E box of the prothymosin-  gene and the coding region of the p15Ink4b gene as negative control  (Staller et al., 2001  ).	bind
15051	1	5410	6	10	NULL	NULL	NULL	CRM1 exportin	GP		bind					IRF-3	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_11_4159_s_174	10805757	(f) CRM1 exportin binding to IRF-3 in vitro.	bind
15300	1	5410	7	10	NULL	NULL	NULL	CRM1 exportin	GP		bind					IRF-3 	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_11_4159_s_174	10805757	(f) CRM1 exportin binding to IRF-3 in vitro.	bind
15052	1	5411	6	10	NULL	NULL	NULL	GTP	Chemical		bind					Rac	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_24_9247_s_214	11094076	(F) EDG5 cells were transiently transfected with expression vectors for myc-tagged wild-type (wt) Rac or V12-Rac and 48 h later were stimulated with S1P (0.1 muM) for 5 min or were not stimulated and assayed for the amounts of GTP-bound forms of Rac and V12-Rac.	bind
15053	2	5411	6	10	NULL	NULL	NULL	GTP	Chemical		bind					Rac	GP		V12		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_24_9247_s_214	11094076	(F) EDG5 cells were transiently transfected with expression vectors for myc-tagged wild-type (wt) Rac or V12-Rac and 48 h later were stimulated with S1P (0.1 muM) for 5 min or were not stimulated and assayed for the amounts of GTP-bound forms of Rac and V12-Rac.	bind
15301	1	5411	7	10	NULL	NULL	NULL	GTP	Chemical		bind					Rac	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_24_9247_s_214	11094076	(F) EDG5 cells were transiently transfected with expression vectors for myc-tagged wild-type (wt) Rac or V12-Rac and 48 h later were stimulated with S1P (0.1 muM) for 5 min or were not stimulated and assayed for the amounts of GTP-bound forms of Rac and V12-Rac.	bind
15302	2	5411	7	10	NULL	NULL	NULL	GTP	Chemical		bind					Rac	GP		V12		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_24_9247_s_214	11094076	(F) EDG5 cells were transiently transfected with expression vectors for myc-tagged wild-type (wt) Rac or V12-Rac and 48 h later were stimulated with S1P (0.1 muM) for 5 min or were not stimulated and assayed for the amounts of GTP-bound forms of Rac and V12-Rac.	bind
15054	1	5412	6	10	NULL	NULL	NULL	CbaR	GP		bind					P cbaA DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_67_8_3530_s_219	11472929	(F) Effects of benzoate and various hydroxylated benzoates on CbaR binding to P cbaA DNA.	bind
15303	1	5412	7	10	NULL	NULL	NULL	CbaR	GP		bind					P cbaA DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_67_8_3530_s_219	11472929	(F) Effects of benzoate and various hydroxylated benzoates on CbaR binding to P cbaA DNA.	bind
15055	1	5413	6	10	NULL	NULL	NULL	Runx2	GP		bind					BSP DNA	NucleicAcid			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_21_9460_s_158	16227596	(F) EMSA used  to test the ability of wild-type Msx2, but not mutant Msx2 (His), to block the binding  of Runx2 to its target DNA derived from the BSP promoter.	bind
15056	2	5413	6	10	NULL	NULL	NULL	Msx2	GP	wild type	block					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_21_9460_s_158	16227596	(F) EMSA used  to test the ability of wild-type Msx2, but not mutant Msx2 (His), to block the binding  of Runx2 to its target DNA derived from the BSP promoter.	bind
15057	3	5413	6	10	NULL	NULL	NULL	Msx2	GP	mutant	does not block					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_21_9460_s_158	16227596	(F) EMSA used  to test the ability of wild-type Msx2, but not mutant Msx2 (His), to block the binding  of Runx2 to its target DNA derived from the BSP promoter.	bind
15304	1	5413	7	10	NULL	NULL	NULL	Runx2	GP		binds					BSP DNA	NucleicAcid			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_21_9460_s_158	16227596	(F) EMSA used  to test the ability of wild-type Msx2, but not mutant Msx2 (His), to block the binding  of Runx2 to its target DNA derived from the BSP promoter.	bind
15305	2	5413	7	10	NULL	NULL	NULL	Msx2	GP	Wild-type	blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_21_9460_s_158	16227596	(F) EMSA used  to test the ability of wild-type Msx2, but not mutant Msx2 (His), to block the binding  of Runx2 to its target DNA derived from the BSP promoter.	bind
53080	3	5413	7	10	NULL	NULL	NULL	Msx2	GP	mutant	does not block					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_21_9460_s_158	16227596	(F) EMSA used  to test the ability of wild-type Msx2, but not mutant Msx2 (His), to block the binding  of Runx2 to its target DNA derived from the BSP promoter.	bind
15058	1	5414	6	10	NULL	NULL	NULL	GRH	GP		bind								FP3 motif		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_4_1434_s_171	16449654	(F) GRH binding to the FP3 motif in a gel shift assay can be deduced from the  competition of the marked shifts by nonoverlapping GRH binding site FP1 (the applied  competitor fragments are referred to by their proximal and distal binding sites and  are indicated above the lanes).	bind
15213	2	5414	6	NULL	NULL	0	NULL		NULL		bind	NULL			GRH binding site FP1		NULL		FP3 motif		NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_4_1434_s_171	16449654	(F) GRH binding to the FP3 motif in a gel shift assay can be deduced from the  competition of the marked shifts by nonoverlapping GRH binding site FP1 (the applied  competitor fragments are referred to by their proximal and distal binding sites and  are indicated above the lanes).	bind
15214	3	5414	6	10	NULL	NULL	NULL	statement 1	Process		competes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_4_1434_s_171	16449654	(F) GRH binding to the FP3 motif in a gel shift assay can be deduced from the  competition of the marked shifts by nonoverlapping GRH binding site FP1 (the applied  competitor fragments are referred to by their proximal and distal binding sites and  are indicated above the lanes).	bind
15306	1	5414	7	10	NULL	NULL	NULL	GRH	GP		bind								 FP3 motif		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_4_1434_s_171	16449654	(F) GRH binding to the FP3 motif in a gel shift assay can be deduced from the  competition of the marked shifts by nonoverlapping GRH binding site FP1 (the applied  competitor fragments are referred to by their proximal and distal binding sites and  are indicated above the lanes).	bind
19993	2	5414	7	NULL	NULL	0	NULL		NULL		bind	NULL			GRH binding site FP1		NULL		FP3 motif		NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_4_1434_s_171	16449654	(F) GRH binding to the FP3 motif in a gel shift assay can be deduced from the  competition of the marked shifts by nonoverlapping GRH binding site FP1 (the applied  competitor fragments are referred to by their proximal and distal binding sites and  are indicated above the lanes).	bind
19994	3	5414	7	10	NULL	NULL	NULL	statement 1	Process		compete with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_4_1434_s_171	16449654	(F) GRH binding to the FP3 motif in a gel shift assay can be deduced from the  competition of the marked shifts by nonoverlapping GRH binding site FP1 (the applied  competitor fragments are referred to by their proximal and distal binding sites and  are indicated above the lanes).	bind
15059	1	5415	6	10	NULL	NULL	NULL	Rho1	GP		bind					alpha-catenin	GP				NULL		NULL	NULL	NULL	NULL	gw60_development_129_16_3771_s_214	12135916	(F) GST pulldown experiments demonstrating the regions of Rho1 required for binding of alpha-catenin (top panel) and p120ctn (second panel from top).	bind
15060	2	5415	6	10	NULL	NULL	NULL	Rho1	GP		bind					p120ctn	GP				NULL		NULL	NULL	NULL	NULL	gw60_development_129_16_3771_s_214	12135916	(F) GST pulldown experiments demonstrating the regions of Rho1 required for binding of alpha-catenin (top panel) and p120ctn (second panel from top).	bind
15307	1	5415	7	10	NULL	NULL	NULL	Rho1	GP		bind					alpha-catenin	GP				NULL		NULL	NULL	NULL	NULL	gw60_development_129_16_3771_s_214	12135916	(F) GST pulldown experiments demonstrating the regions of Rho1 required for binding of alpha-catenin (top panel) and p120ctn (second panel from top).	bind
15308	2	5415	7	10	NULL	NULL	NULL	Rho1	GP		bind					 p120ctn	GP				NULL		NULL	NULL	NULL	NULL	gw60_development_129_16_3771_s_214	12135916	(F) GST pulldown experiments demonstrating the regions of Rho1 required for binding of alpha-catenin (top panel) and p120ctn (second panel from top).	bind
15061	1	5416	6	10	NULL	NULL	NULL	IGF-I	GP		induces					Shc	GP	phosphorylation of			NULL	Shc-3F - expressing cells	NULL	NULL	NULL	NULL	gw70_molbiolcell_16_7_3353_s_177	15888547	(F) IGF-I - induced Shc phosphorylation and Shc  binding to Grb2 as well as phosphorylation of Erk1,2 in vector and in Shc-3F - expressing  cells are shown.	bind
15062	2	5416	6	10	NULL	NULL	NULL	Shc	GP		bind					Grb2	GP				NULL	Shc-3F - expressing cells	NULL	NULL	NULL	NULL	gw70_molbiolcell_16_7_3353_s_177	15888547	(F) IGF-I - induced Shc phosphorylation and Shc  binding to Grb2 as well as phosphorylation of Erk1,2 in vector and in Shc-3F - expressing  cells are shown.	bind
15063	3	5416	6	10	NULL	NULL	NULL	IGF-I	GP		induces					statement 2	Process				NULL	Shc-3F - expressing cells	NULL	NULL	NULL	NULL	gw70_molbiolcell_16_7_3353_s_177	15888547	(F) IGF-I - induced Shc phosphorylation and Shc  binding to Grb2 as well as phosphorylation of Erk1,2 in vector and in Shc-3F - expressing  cells are shown.	bind
15064	4	5416	6	10	NULL	NULL	NULL	IGF-I	GP		induces					Erk1/2	GP	phosphorylation of			NULL	Shc-3F - expressing cells	NULL	NULL	NULL	NULL	gw70_molbiolcell_16_7_3353_s_177	15888547	(F) IGF-I - induced Shc phosphorylation and Shc  binding to Grb2 as well as phosphorylation of Erk1,2 in vector and in Shc-3F - expressing  cells are shown.	bind
15309	1	5416	7	10	NULL	NULL	NULL	Shc	GP		bind					Grb2	GP				NULL	Shc-3F - expressing cells	NULL	NULL	NULL	NULL	gw70_molbiolcell_16_7_3353_s_177	15888547	(F) IGF-I - induced Shc phosphorylation and Shc  binding to Grb2 as well as phosphorylation of Erk1,2 in vector and in Shc-3F - expressing  cells are shown.	bind
15310	2	5416	7	10	NULL	NULL	NULL	IGF-I 	GP		induce					statement 1	Process				NULL	Shc-3F - expressing cells	NULL	NULL	NULL	NULL	gw70_molbiolcell_16_7_3353_s_177	15888547	(F) IGF-I - induced Shc phosphorylation and Shc  binding to Grb2 as well as phosphorylation of Erk1,2 in vector and in Shc-3F - expressing  cells are shown.	bind
15311	3	5416	7	10	NULL	NULL	NULL	IGF-I	GP		induce					Shc	GP	phosphorylation of			NULL	Shc-3F - expressing cells	NULL	NULL	NULL	NULL	gw70_molbiolcell_16_7_3353_s_177	15888547	(F) IGF-I - induced Shc phosphorylation and Shc  binding to Grb2 as well as phosphorylation of Erk1,2 in vector and in Shc-3F - expressing  cells are shown.	bind
15313	5	5416	7	10	NULL	NULL	NULL	IGF-I	GP		induce					Erk1,2	GP	phosphorylation of			NULL	Shc-3F - expressing cells	NULL	NULL	NULL	NULL	gw70_molbiolcell_16_7_3353_s_177	15888547	(F) IGF-I - induced Shc phosphorylation and Shc  binding to Grb2 as well as phosphorylation of Erk1,2 in vector and in Shc-3F - expressing  cells are shown.	bind
15065	1	5418	6	10	NULL	NULL	NULL	KSRP	GP		bind					fos RNA	NucleicAcid			ARE	NULL		NULL	NULL	NULL	NULL	gw60_cell_107_4_451_s_227	11719186	(F) KSRP binds AREfos RNA.	bind
15315	1	5418	7	10	NULL	NULL	NULL	KSRP	GP		binds					fos RNA	NucleicAcid			ARE	NULL		NULL	NULL	NULL	NULL	gw60_cell_107_4_451_s_227	11719186	(F) KSRP binds AREfos RNA.	bind
15066	1	5420	6	10	NULL	NULL	NULL	Myosin-I	GP		does not bind					syntaxin-1A	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_103	16030255	(F) Myosin-I (myr1A) and myosin-IIB do  not bind to syntaxin-1A, even though they are present in the brain homogenate.	bind
15067	2	5420	6	10	NULL	NULL	NULL	myosin-IIB	GP		does not bind					syntaxin-1A	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_103	16030255	(F) Myosin-I (myr1A) and myosin-IIB do  not bind to syntaxin-1A, even though they are present in the brain homogenate.	bind
19040	3	5420	6	10	NULL	NULL	NULL	Myosin-I	GP		is					myr1A	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_103	16030255	(F) Myosin-I (myr1A) and myosin-IIB do  not bind to syntaxin-1A, even though they are present in the brain homogenate.	bind
15316	1	5420	7	10	NULL	NULL	NULL	Myosin-I	GP		does not bind					syntaxin-1A	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_103	16030255	(F) Myosin-I (myr1A) and myosin-IIB do  not bind to syntaxin-1A, even though they are present in the brain homogenate.	bind
15319	2	5420	7	10	NULL	NULL	NULL	myosin-IIB	GP		does not bind					syntaxin-1A	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_103	16030255	(F) Myosin-I (myr1A) and myosin-IIB do  not bind to syntaxin-1A, even though they are present in the brain homogenate.	bind
15321	3	5420	7	10	NULL	NULL	NULL	Myosin-I	GP		is					myr1A	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4519_s_103	16030255	(F) Myosin-I (myr1A) and myosin-IIB do  not bind to syntaxin-1A, even though they are present in the brain homogenate.	bind
15068	2	5421	6	10	NULL	NULL	NULL	p53	GP		bind					statement 2	Process				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_2014_s_359	15713654	(F) p53 and p53(deltaAD1deltaBD) bind the p53-responsive element within the p21 promoter in vivo.	bind
15069	3	5421	6	10	NULL	NULL	NULL	p53	GP		bind			deltaAD1deltaBD		statement 1	Process				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_2014_s_359	15713654	(F) p53 and p53(deltaAD1deltaBD) bind the p53-responsive element within the p21 promoter in vivo.	bind
53087	1	5421	6	10	NULL	NULL	NULL				resides within				p53-responsive element	p21	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_2014_s_359	15713654	(F) p53 and p53(deltaAD1deltaBD) bind the p53-responsive element within the p21 promoter in vivo.	bind
15323	2	5421	7	10	NULL	NULL	NULL	p53	GP		bind					statement 1	Process				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_2014_s_359	15713654	(F) p53 and p53(deltaAD1deltaBD) bind the p53-responsive element within the p21 promoter in vivo.	bind
15325	3	5421	7	10	NULL	NULL	NULL	 p53	GP		bind			deltaAD1deltaBD		statement 1	Process			 	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_2014_s_359	15713654	(F) p53 and p53(deltaAD1deltaBD) bind the p53-responsive element within the p21 promoter in vivo.	bind
53088	1	5421	7	10	NULL	NULL	NULL				resides within				p53-responsive element	p21	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_2014_s_359	15713654	(F) p53 and p53(deltaAD1deltaBD) bind the p53-responsive element within the p21 promoter in vivo.	bind
15070	1	5422	6	10	NULL	NULL	NULL	AGAP1	GP		bind			PH domain		AP-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_5_3_513_s_58	12967569	(F) PH domain of AGAP1 binds to AP-3.	bind
15328	1	5422	7	10	NULL	NULL	NULL	AGAP1	GP		bind			PH domain		AP-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_5_3_513_s_58	12967569	(F) PH domain of AGAP1 binds to AP-3.	bind
15071	1	5423	6	10	NULL	NULL	NULL	HDAC1	GP		bind					bcl-2	GP			P2 promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1608_s_290	15713621	(F) Quantitative ChIP assays of the binding of HDAC1 and HDAC2 to the  bcl-2 P2 promoter.	bind
15072	2	5423	6	10	NULL	NULL	NULL	HDAC2	GP		bind					bcl-2	GP			P2 promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1608_s_290	15713621	(F) Quantitative ChIP assays of the binding of HDAC1 and HDAC2 to the  bcl-2 P2 promoter.	bind
15331	1	5423	7	10	NULL	NULL	NULL	 HDAC1	GP		bind					bcl-2 	GP			P2 promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1608_s_290	15713621	(F) Quantitative ChIP assays of the binding of HDAC1 and HDAC2 to the  bcl-2 P2 promoter.	bind
15332	2	5423	7	10	NULL	NULL	NULL	HDAC2 	GP		bind					bcl-2 	GP			P2 promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1608_s_290	15713621	(F) Quantitative ChIP assays of the binding of HDAC1 and HDAC2 to the  bcl-2 P2 promoter.	bind
15073	2	5424	6	10	NULL	NULL	NULL	Brg	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_19_2_169_s_177	12932351	(F) Real-time PCR quantifying the binding of Brg to the proximal  TCF site at the  Myc promoter.	bind
53089	1	5424	6	10	NULL	NULL	NULL			proximal	resides within				TCF site	Myc	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_immunity_19_2_169_s_177	12932351	(F) Real-time PCR quantifying the binding of Brg to the proximal  TCF site at the  Myc promoter.	bind
15333	2	5424	7	10	NULL	NULL	NULL	Brg 	GP 		bind					statement 1	Process			 	NULL		NULL	NULL	NULL	NULL	gw60_immunity_19_2_169_s_177	12932351	(F) Real-time PCR quantifying the binding of Brg to the proximal  TCF site at the  Myc promoter.	bind
53090	1	5424	7	10	NULL	NULL	NULL			proximal	resides within				TCF site	Myc	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_immunity_19_2_169_s_177	12932351	(F) Real-time PCR quantifying the binding of Brg to the proximal  TCF site at the  Myc promoter.	bind
15215	1	5425	6	10	NULL	NULL	NULL	ApoER2-Fc	GP		bind					protein A	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_24_2_481_s_72	10571241	(F) Recombinant Fc fusion proteins from 1 ml 293 culture supernatant transfected (lanes 1-5) or not transfected (lane 6) with the ApoER2-Fc expression plasmid were bound to 40  l protein A Sepharose slurry, followed by incubation with 500  l Reelin containing (lanes 1-4 and 6) or not containing (lane 5) 293 cell culture supernatant without additions (lane 1) or in the presence of 30  g/ml GST-RAP (lane 2), 30  g/ml GST (lane 3), or 30 mM EDTA (lane 4).	bind
15334	1	5425	7	10	NULL	NULL	NULL	ApoER2-Fc	GP		bind					 protein A 	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_24_2_481_s_72	10571241	(F) Recombinant Fc fusion proteins from 1 ml 293 culture supernatant transfected (lanes 1-5) or not transfected (lane 6) with the ApoER2-Fc expression plasmid were bound to 40  l protein A Sepharose slurry, followed by incubation with 500  l Reelin containing (lanes 1-4 and 6) or not containing (lane 5) 293 cell culture supernatant without additions (lane 1) or in the presence of 30  g/ml GST-RAP (lane 2), 30  g/ml GST (lane 3), or 30 mM EDTA (lane 4).	bind
15074	1	5426	6	10	NULL	NULL	NULL	RF-Cp145	GP		bind			domain B		GST-Rb	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_4_715_s_107	11336696	(F) RF-Cp145 domain B binds to GST-Rb in an LxCxE-dependent manner.	bind
15075	2	5426	6	10	NULL	NULL	NULL	statement 1	Process		is dependent on								LxCxE		NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_4_715_s_107	11336696	(F) RF-Cp145 domain B binds to GST-Rb in an LxCxE-dependent manner.	bind
15335	1	5426	7	10	NULL	NULL	NULL	RF-Cp145	GP		binds to			domain B		GST-Rb	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_4_715_s_107	11336696	(F) RF-Cp145 domain B binds to GST-Rb in an LxCxE-dependent manner.	bind
15336	2	5426	7	10	NULL	NULL	NULL	statement 1	Process		depends on								LxCxE		NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_4_715_s_107	11336696	(F) RF-Cp145 domain B binds to GST-Rb in an LxCxE-dependent manner.	bind
15076	1	5427	6	10	NULL	NULL	NULL	NAF1	GP		bind					NAP57	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_2_207_s_50	16618814	(F) Schematic depiction  of the mutually exclusive binding of NAF1 and GAR1 to NAP57 in the context of the  core trimer.	bind
15077	2	5427	6	10	NULL	NULL	NULL	GAR1	GP		bind					NAP57	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_2_207_s_50	16618814	(F) Schematic depiction  of the mutually exclusive binding of NAF1 and GAR1 to NAP57 in the context of the  core trimer.	bind
15078	3	5427	6	10	NULL	NULL	NULL	statement 1	Process		mutually exclusive to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_2_207_s_50	16618814	(F) Schematic depiction  of the mutually exclusive binding of NAF1 and GAR1 to NAP57 in the context of the  core trimer.	bind
15337	1	5427	7	10	NULL	NULL	NULL	NAF1	GP		bind					NAP57	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_2_207_s_50	16618814	(F) Schematic depiction  of the mutually exclusive binding of NAF1 and GAR1 to NAP57 in the context of the  core trimer.	bind
15338	2	5427	7	10	NULL	NULL	NULL	GAR1	GP		bind					NAP57	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_2_207_s_50	16618814	(F) Schematic depiction  of the mutually exclusive binding of NAF1 and GAR1 to NAP57 in the context of the  core trimer.	bind
15339	3	5427	7	10	NULL	NULL	NULL	statement 1	Process		is mutually exclusive to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_2_207_s_50	16618814	(F) Schematic depiction  of the mutually exclusive binding of NAF1 and GAR1 to NAP57 in the context of the  core trimer.	bind
15079	1	5428	6	10	NULL	NULL	NULL	Sec23/24	GP		bind					Sec22	GP	intact			NULL		NULL	NULL	NULL	NULL	gw60_cell_114_4_483_s_49	12941276	(F) Sec23/24 binds to intact Sec22, but not to Bos1.	bind
15080	2	5428	6	10	NULL	NULL	NULL	Sec23/24	GP		does not bind					Bos1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_4_483_s_49	12941276	(F) Sec23/24 binds to intact Sec22, but not to Bos1.	bind
15340	1	5428	7	10	NULL	NULL	NULL	Sec23/24	GP		bind					Sec22	GP	intact			NULL		NULL	NULL	NULL	NULL	gw60_cell_114_4_483_s_49	12941276	(F) Sec23/24 binds to intact Sec22, but not to Bos1.	bind
15341	2	5428	7	10	NULL	NULL	NULL	Sec23/24	GP		does not bind					Bos1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_4_483_s_49	12941276	(F) Sec23/24 binds to intact Sec22, but not to Bos1.	bind
15081	1	5429	6	10	NULL	NULL	NULL	GDP	Chemical		bind					gamma-tubulin	GP				NULL	gammaTuSC	NULL	NULL	NULL	NULL	gw60_cellbiol_144_4_721_s_383	10037793	(F) Small  amounts of both GDP and GTP are detected bound to gamma-tubulin in the gammaTuSC (for quantitation see Table  II: 20 muM GTP, experiment  1).	bind
15082	2	5429	6	10	NULL	NULL	NULL	GTP	Chemical		bind					gamma-tubulin	GP				NULL	gammaTuSC	NULL	NULL	NULL	NULL	gw60_cellbiol_144_4_721_s_383	10037793	(F) Small  amounts of both GDP and GTP are detected bound to gamma-tubulin in the gammaTuSC (for quantitation see Table  II: 20 muM GTP, experiment  1).	bind
15342	1	5429	7	10	NULL	NULL	NULL	GDP	Chemical		bind					gamma-tubulin	GP				NULL	in gammaTuSC	NULL	NULL	NULL	NULL	gw60_cellbiol_144_4_721_s_383	10037793	(F) Small  amounts of both GDP and GTP are detected bound to gamma-tubulin in the gammaTuSC (for quantitation see Table  II: 20 muM GTP, experiment  1).	bind
15343	2	5429	7	10	NULL	NULL	NULL	GTP	Chemical		bind					gamma-tubulin	GP				NULL	in gammaTuSC	NULL	NULL	NULL	NULL	gw60_cellbiol_144_4_721_s_383	10037793	(F) Small  amounts of both GDP and GTP are detected bound to gamma-tubulin in the gammaTuSC (for quantitation see Table  II: 20 muM GTP, experiment  1).	bind
19041	1	5430	6	10	NULL	NULL	NULL	RII	GP	recombinant	bind					Rab32	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_158_4_659_s_70	12186851	(F) Solution binding of recombinant RII and Rab32.	bind
15344	1	5430	7	10	NULL	NULL	NULL	 RII	GP	recombinant	bind					Rab32	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_158_4_659_s_70	12186851	(F) Solution binding of recombinant RII and Rab32.	bind
15216	1	5431	6	10	NULL	NULL	NULL	Gfi1	GP	silencing of	diminishes					G9a	GP	binding of			NULL	HL-60 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10338_s_287	16287849	(F) Specific silencing of Gfi1 by siRNA, but [[ not nonspecific  control ]] siRNA (as shown by Western blotting, right panel), diminishes binding of  G9a and HDAC1, diminishes incorporation of dimethylated histone H3-K9, and modestly  increases incorporation of AcyH3, on the p21Cip/WAF1 promoter in HL-60 cells (as revealed by ChIP, left and middle panels).	bind
15217	2	5431	6	10	NULL	NULL	NULL	AcyH3	GP		incorporated on					p21Cip/WAF1	GP			promoter	NULL	HL-60 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10338_s_287	16287849	(F) Specific silencing of Gfi1 by siRNA, but [[ not nonspecific  control ]] siRNA (as shown by Western blotting, right panel), diminishes binding of  G9a and HDAC1, diminishes incorporation of dimethylated histone H3-K9, and modestly  increases incorporation of AcyH3, on the p21Cip/WAF1 promoter in HL-60 cells (as revealed by ChIP, left and middle panels).	bind
15218	3	5431	6	10	NULL	NULL	NULL	histone H3-K9	GP	dimethylated	incorporated on					p21Cip/WAF1	GP			promoter	NULL	HL-60 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10338_s_287	16287849	(F) Specific silencing of Gfi1 by siRNA, but [[ not nonspecific  control ]] siRNA (as shown by Western blotting, right panel), diminishes binding of  G9a and HDAC1, diminishes incorporation of dimethylated histone H3-K9, and modestly  increases incorporation of AcyH3, on the p21Cip/WAF1 promoter in HL-60 cells (as revealed by ChIP, left and middle panels).	bind
15219	4	5431	6	10	NULL	NULL	NULL	Gfi1	GP	silencing of	diminishes					HDAC1	GP	binding of			NULL	HL-60 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10338_s_287	16287849	(F) Specific silencing of Gfi1 by siRNA, but [[ not nonspecific  control ]] siRNA (as shown by Western blotting, right panel), diminishes binding of  G9a and HDAC1, diminishes incorporation of dimethylated histone H3-K9, and modestly  increases incorporation of AcyH3, on the p21Cip/WAF1 promoter in HL-60 cells (as revealed by ChIP, left and middle panels).	bind
15220	5	5431	6	10	NULL	NULL	NULL	Gfi1	GP	silencing of	diminishes					statement 3	Process				NULL	HL-60 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10338_s_287	16287849	(F) Specific silencing of Gfi1 by siRNA, but [[ not nonspecific  control ]] siRNA (as shown by Western blotting, right panel), diminishes binding of  G9a and HDAC1, diminishes incorporation of dimethylated histone H3-K9, and modestly  increases incorporation of AcyH3, on the p21Cip/WAF1 promoter in HL-60 cells (as revealed by ChIP, left and middle panels).	bind
15221	6	5431	6	10	NULL	NULL	NULL	Gfi1	GP	silencing of	increases		modestly			statement 2	Process				NULL	HL-60 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10338_s_287	16287849	(F) Specific silencing of Gfi1 by siRNA, but [[ not nonspecific  control ]] siRNA (as shown by Western blotting, right panel), diminishes binding of  G9a and HDAC1, diminishes incorporation of dimethylated histone H3-K9, and modestly  increases incorporation of AcyH3, on the p21Cip/WAF1 promoter in HL-60 cells (as revealed by ChIP, left and middle panels).	bind
15345	1	5431	7	10	NULL	NULL	NULL	Gfi1	GP	silencing of	diminishes					G9a	GP	binding of			NULL	HL-60 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10338_s_287	16287849	(F) Specific silencing of Gfi1 by siRNA, but [[ not nonspecific  control ]] siRNA (as shown by Western blotting, right panel), diminishes binding of  G9a and HDAC1, diminishes incorporation of dimethylated histone H3-K9, and modestly  increases incorporation of AcyH3, on the p21Cip/WAF1 promoter in HL-60 cells (as revealed by ChIP, left and middle panels).	bind
15346	2	5431	7	10	NULL	NULL	NULL	Gfi1	GP	silencing of	diminishes					HDAC1	GP	binding of			NULL	HL-60 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10338_s_287	16287849	(F) Specific silencing of Gfi1 by siRNA, but [[ not nonspecific  control ]] siRNA (as shown by Western blotting, right panel), diminishes binding of  G9a and HDAC1, diminishes incorporation of dimethylated histone H3-K9, and modestly  increases incorporation of AcyH3, on the p21Cip/WAF1 promoter in HL-60 cells (as revealed by ChIP, left and middle panels).	bind
15347	3	5431	7	10	NULL	NULL	NULL	AcyH3	GP		incorporated on					p21Cip/WAF1	GP			promoter	NULL	HL-60 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10338_s_287	16287849	(F) Specific silencing of Gfi1 by siRNA, but [[ not nonspecific  control ]] siRNA (as shown by Western blotting, right panel), diminishes binding of  G9a and HDAC1, diminishes incorporation of dimethylated histone H3-K9, and modestly  increases incorporation of AcyH3, on the p21Cip/WAF1 promoter in HL-60 cells (as revealed by ChIP, left and middle panels).	bind
15348	5	5431	7	10	NULL	NULL	NULL	histone H3-K9	GP	dimethylated	incorporated on					p21Cip/WAF1	GP			promoter	NULL	HL-60 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10338_s_287	16287849	(F) Specific silencing of Gfi1 by siRNA, but [[ not nonspecific  control ]] siRNA (as shown by Western blotting, right panel), diminishes binding of  G9a and HDAC1, diminishes incorporation of dimethylated histone H3-K9, and modestly  increases incorporation of AcyH3, on the p21Cip/WAF1 promoter in HL-60 cells (as revealed by ChIP, left and middle panels).	bind
53091	4	5431	7	10	NULL	NULL	NULL	Gfi1	GP	silencing of	diminishes					statement 3	Process				NULL	HL-60 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10338_s_287	16287849	(F) Specific silencing of Gfi1 by siRNA, but [[ not nonspecific  control ]] siRNA (as shown by Western blotting, right panel), diminishes binding of  G9a and HDAC1, diminishes incorporation of dimethylated histone H3-K9, and modestly  increases incorporation of AcyH3, on the p21Cip/WAF1 promoter in HL-60 cells (as revealed by ChIP, left and middle panels).	bind
53092	6	5431	7	10	NULL	NULL	NULL	Gfi1	GP	silencing of	diminishes					statement 5	Process				NULL	HL-60 cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10338_s_287	16287849	(F) Specific silencing of Gfi1 by siRNA, but [[ not nonspecific  control ]] siRNA (as shown by Western blotting, right panel), diminishes binding of  G9a and HDAC1, diminishes incorporation of dimethylated histone H3-K9, and modestly  increases incorporation of AcyH3, on the p21Cip/WAF1 promoter in HL-60 cells (as revealed by ChIP, left and middle panels).	bind
15222	1	5433	6	10	NULL	NULL	NULL	nucleoporin repeats	GP		bind			x-Phe-Gly residues		TAP	GP		NTF2-like domain		NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_3_645_s_135	11583626	(F) Superposition of the x-Phe-Gly residues of nucleoporin repeats bound to TAP NTF2-like domain (black) and to importin   (gray;  Bayliss et al., 2000  ) shows they have a similar conformation when bound to the two different transport factors.	bind
15223	2	5433	6	10	NULL	NULL	NULL	nucleoporin repeats	GP		bind			x-Phe-Gly residues		importin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_3_645_s_135	11583626	(F) Superposition of the x-Phe-Gly residues of nucleoporin repeats bound to TAP NTF2-like domain (black) and to importin   (gray;  Bayliss et al., 2000  ) shows they have a similar conformation when bound to the two different transport factors.	bind
15349	1	5433	7	10	NULL	NULL	NULL	nucleoporin repeats	GP		bind			x-Phe-Gly residues		TAP	GP		NTF2-like domain		NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_3_645_s_135	11583626	(F) Superposition of the x-Phe-Gly residues of nucleoporin repeats bound to TAP NTF2-like domain (black) and to importin   (gray;  Bayliss et al., 2000  ) shows they have a similar conformation when bound to the two different transport factors.	bind
15350	2	5433	7	10	NULL	NULL	NULL	 nucleoporin repeats	GP		bind			x-Phe-Gly residues		importin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_3_645_s_135	11583626	(F) Superposition of the x-Phe-Gly residues of nucleoporin repeats bound to TAP NTF2-like domain (black) and to importin   (gray;  Bayliss et al., 2000  ) shows they have a similar conformation when bound to the two different transport factors.	bind
15083	1	5434	6	10	NULL	NULL	NULL	eIF2B	GP		bind					eIF2alpha	GP	phosphorylated			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3063_s_337	15798194	(F) Surface representation of eIF2alpha highlighting residues (purple) important for binding and inhibition of eIF2B by phosphorylated  eIF2alpha.	bind
15084	2	5434	6	10	NULL	NULL	NULL	eIF2alpha	GP	phosphorylated	inhibits					eIF2B	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3063_s_337	15798194	(F) Surface representation of eIF2alpha highlighting residues (purple) important for binding and inhibition of eIF2B by phosphorylated  eIF2alpha.	bind
15351	1	5434	7	10	NULL	NULL	NULL	eIF2alpha	GP	phosphorylated	bind					eIF2B	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3063_s_337	15798194	(F) Surface representation of eIF2alpha highlighting residues (purple) important for binding and inhibition of eIF2B by phosphorylated  eIF2alpha.	bind
15352	2	5434	7	10	NULL	NULL	NULL	eIF2alpha	GP	phosphorylated	inhibits					eIF2B	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3063_s_337	15798194	(F) Surface representation of eIF2alpha highlighting residues (purple) important for binding and inhibition of eIF2B by phosphorylated  eIF2alpha.	bind
15224	1	5435	6	10	NULL	NULL	NULL	TAL1beta-BM	GP		induces					RALDH2-T	GP	endogenous expression of			NULL	HPB-ALL cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6939_s_307	9819382	(F) TAL1beta-BM induces endogeneous  RALDH2-T expression with LMO in HPB-ALL cells.	bind
15225	2	5435	6	10	NULL	NULL	NULL	statement 1	Process		occurs with					LMO	GP				NULL	HPB-ALL cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6939_s_307	9819382	(F) TAL1beta-BM induces endogeneous  RALDH2-T expression with LMO in HPB-ALL cells.	bind
15353	1	5435	7	10	NULL	NULL	NULL	TAL1beta-BM	GP		induces					RALDH2-T	GP	endogenous expression of			NULL	HPB-ALL cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6939_s_307	9819382	(F) TAL1beta-BM induces endogeneous  RALDH2-T expression with LMO in HPB-ALL cells.	bind
15394	2	5435	7	10	NULL	NULL	NULL	statement 1	Process		occurs with					LMO	GP				NULL	HPB-ALL cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6939_s_307	9819382	(F) TAL1beta-BM induces endogeneous  RALDH2-T expression with LMO in HPB-ALL cells.	bind
15085	1	5436	6	10	NULL	NULL	NULL	HDAC1	GP		bind					GST-Rb	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_142	15485920	(F) The  Raf-1 peptide specifically disrupts the Rb-Raf-1 interaction but does not affect  the binding of HDAC1, cyclin D, and prohibitin to GST-Rb.	bind
15086	2	5436	6	10	NULL	NULL	NULL	cyclin D	GP		bind					GST-Rb	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_142	15485920	(F) The  Raf-1 peptide specifically disrupts the Rb-Raf-1 interaction but does not affect  the binding of HDAC1, cyclin D, and prohibitin to GST-Rb.	bind
15087	3	5436	6	10	NULL	NULL	NULL	Prohibitin	GP		bind					GST-Rb	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_142	15485920	(F) The  Raf-1 peptide specifically disrupts the Rb-Raf-1 interaction but does not affect  the binding of HDAC1, cyclin D, and prohibitin to GST-Rb.	bind
15088	4	5436	6	10	NULL	NULL	NULL	Raf-1 peptide	GP		does not affect					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_142	15485920	(F) The  Raf-1 peptide specifically disrupts the Rb-Raf-1 interaction but does not affect  the binding of HDAC1, cyclin D, and prohibitin to GST-Rb.	bind
15089	5	5436	6	10	NULL	NULL	NULL	Raf-1 peptide	GP		does not affect					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_142	15485920	(F) The  Raf-1 peptide specifically disrupts the Rb-Raf-1 interaction but does not affect  the binding of HDAC1, cyclin D, and prohibitin to GST-Rb.	bind
15090	6	5436	6	10	NULL	NULL	NULL	Raf-1 peptide	GP		does not affect					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_142	15485920	(F) The  Raf-1 peptide specifically disrupts the Rb-Raf-1 interaction but does not affect  the binding of HDAC1, cyclin D, and prohibitin to GST-Rb.	bind
15091	7	5436	6	10	NULL	NULL	NULL	Raf-1 peptide	GP		disrupts		specifically			Rb-Raf-1	GP	interaction of 			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_142	15485920	(F) The  Raf-1 peptide specifically disrupts the Rb-Raf-1 interaction but does not affect  the binding of HDAC1, cyclin D, and prohibitin to GST-Rb.	bind
15477	1	5436	7	10	NULL	NULL	NULL	Raf-1 peptide	GP		disrupts		specifically			Rb-Raf-1	GP	interaction of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_142	15485920	(F) The  Raf-1 peptide specifically disrupts the Rb-Raf-1 interaction but does not affect  the binding of HDAC1, cyclin D, and prohibitin to GST-Rb.	bind
15478	2	5436	7	10	NULL	NULL	NULL	HDAC1	GP		bind					GST-Rb	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_142	15485920	(F) The  Raf-1 peptide specifically disrupts the Rb-Raf-1 interaction but does not affect  the binding of HDAC1, cyclin D, and prohibitin to GST-Rb.	bind
15479	3	5436	7	10	NULL	NULL	NULL	 cyclin D	GP		bind					GST-Rb	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_142	15485920	(F) The  Raf-1 peptide specifically disrupts the Rb-Raf-1 interaction but does not affect  the binding of HDAC1, cyclin D, and prohibitin to GST-Rb.	bind
15480	4	5436	7	10	NULL	NULL	NULL	prohibitin	GP		binds					GST-Rb	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_142	15485920	(F) The  Raf-1 peptide specifically disrupts the Rb-Raf-1 interaction but does not affect  the binding of HDAC1, cyclin D, and prohibitin to GST-Rb.	bind
15481	5	5436	7	10	NULL	NULL	NULL	Raf-1 peptide	GP		does not affect					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_142	15485920	(F) The  Raf-1 peptide specifically disrupts the Rb-Raf-1 interaction but does not affect  the binding of HDAC1, cyclin D, and prohibitin to GST-Rb.	bind
15482	6	5436	7	10	NULL	NULL	NULL	Raf-1 peptide	GP		does not affect					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_142	15485920	(F) The  Raf-1 peptide specifically disrupts the Rb-Raf-1 interaction but does not affect  the binding of HDAC1, cyclin D, and prohibitin to GST-Rb.	bind
15483	7	5436	7	10	NULL	NULL	NULL	Raf-1 peptide	GP		does not affect					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_142	15485920	(F) The  Raf-1 peptide specifically disrupts the Rb-Raf-1 interaction but does not affect  the binding of HDAC1, cyclin D, and prohibitin to GST-Rb.	bind
15092	1	5437	6	10	NULL	NULL	NULL	ATM	GP		bind					plasmid DNA	NucleicAcid	linearized			NULL	Nbs1-depleted extract	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5363_s_336	15964794	(F) The C147 fragment  of Nbs1 restores ATM binding to linearized plasmid DNA and damaged sperm chromatin  in an Nbs1-depleted extract.	bind
15093	2	5437	6	10	NULL	NULL	NULL	ATM	GP		bind					sperm chromatin	Chromosome	damaged			NULL	Nbs1-depleted extract	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5363_s_336	15964794	(F) The C147 fragment  of Nbs1 restores ATM binding to linearized plasmid DNA and damaged sperm chromatin  in an Nbs1-depleted extract.	bind
15094	3	5437	6	10	NULL	NULL	NULL	Nbs1	GP		restores			C147 fragment		statement 1	Process				NULL	Nbs1-depleted extract	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5363_s_336	15964794	(F) The C147 fragment  of Nbs1 restores ATM binding to linearized plasmid DNA and damaged sperm chromatin  in an Nbs1-depleted extract.	bind
15095	4	5437	6	10	NULL	NULL	NULL	Nbs1	GP		restores			C147 fragment		statement 2	Process				NULL	Nbs1-depleted extract	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5363_s_336	15964794	(F) The C147 fragment  of Nbs1 restores ATM binding to linearized plasmid DNA and damaged sperm chromatin  in an Nbs1-depleted extract.	bind
15484	1	5437	7	10	NULL	NULL	NULL	ATM	GP		bind					plasmid DNA	NucleicAcid	 linearized			NULL	Nbs1-depleted extract	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5363_s_336	15964794	(F) The C147 fragment  of Nbs1 restores ATM binding to linearized plasmid DNA and damaged sperm chromatin  in an Nbs1-depleted extract.	bind
15485	2	5437	7	10	NULL	NULL	NULL	ATM	GP		bind					sperm chromatin	Chromosome	damaged			NULL	Nbs1-depleted extract	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5363_s_336	15964794	(F) The C147 fragment  of Nbs1 restores ATM binding to linearized plasmid DNA and damaged sperm chromatin  in an Nbs1-depleted extract.	bind
15486	3	5437	7	10	NULL	NULL	NULL	Nbs1	GP		restores			 C147 fragment		statement 1	Process				NULL	Nbs1-depleted extract	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5363_s_336	15964794	(F) The C147 fragment  of Nbs1 restores ATM binding to linearized plasmid DNA and damaged sperm chromatin  in an Nbs1-depleted extract.	bind
15487	4	5437	7	10	NULL	NULL	NULL	Nbs1	GP		restores			C147 fragment		statement 2	Process				NULL	Nbs1-depleted extract	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5363_s_336	15964794	(F) The C147 fragment  of Nbs1 restores ATM binding to linearized plasmid DNA and damaged sperm chromatin  in an Nbs1-depleted extract.	bind
15096	1	5438	6	10	NULL	NULL	NULL	GST-Jun proteins	GP		bind					JNK	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_87_5_929_s_109	8945519	(F) The different GST - Jun  proteins bind JNK.	bind
15488	1	5438	7	10	NULL	NULL	NULL	GST - Jun proteins	GP		bind					JNK	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_87_5_929_s_109	8945519	(F) The different GST - Jun  proteins bind JNK.	bind
15097	1	5441	6	10	NULL	NULL	NULL	lck-GFP D10 cell	Cell		forms a conjugate with					TR-transferrin	GP	internalized			NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_6_809_s_290	12479826	(F) Time points from conjugate formation of an lck-GFP D10 cell with internalized TR-transferrin.	bind
15599	1	5441	7	10	NULL	NULL	NULL	lck-GFP D10 cell	Cell		forms a conjugate with					TR-transferrin	GP	 internalized 			NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_6_809_s_290	12479826	(F) Time points from conjugate formation of an lck-GFP D10 cell with internalized TR-transferrin.	bind
15098	1	5442	6	10	NULL	NULL	NULL	MAE	GP		bind					PNT-P2	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_130_5_845_s_345	12538513	(F) To prevent runaway signaling, a negative feedback loop may  occur in which MAE binds to PNT-P2 and inhibits transcriptional activation.	bind
15099	2	5442	6	10	NULL	NULL	NULL	statement 1	Process		inhibits					transcription	Process	activation of			NULL		NULL	NULL	NULL	NULL	gw70_development_130_5_845_s_345	12538513	(F) To prevent runaway signaling, a negative feedback loop may  occur in which MAE binds to PNT-P2 and inhibits transcriptional activation.	bind
19042	3	5442	6	10	NULL	NULL	NULL	negative feedback loop	Process		lead to 		may 			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_130_5_845_s_345	12538513	(F) To prevent runaway signaling, a negative feedback loop may  occur in which MAE binds to PNT-P2 and inhibits transcriptional activation.	bind
15489	1	5442	7	10	NULL	NULL	NULL	MAE	GP		binds					PNT-P2	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_130_5_845_s_345	12538513	(F) To prevent runaway signaling, a negative feedback loop may  occur in which MAE binds to PNT-P2 and inhibits transcriptional activation.	bind
15490	2	5442	7	10	NULL	NULL	NULL	negative feedback loop	GP		lead to		may			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_130_5_845_s_345	12538513	(F) To prevent runaway signaling, a negative feedback loop may  occur in which MAE binds to PNT-P2 and inhibits transcriptional activation.	bind
15491	3	5442	7	10	NULL	NULL	NULL	statement 1	Process		inhibits					transcription 	Process	activation of			NULL		NULL	NULL	NULL	NULL	gw70_development_130_5_845_s_345	12538513	(F) To prevent runaway signaling, a negative feedback loop may  occur in which MAE binds to PNT-P2 and inhibits transcriptional activation.	bind
15100	1	5444	6	10	NULL	NULL	NULL	CRF	GP		bind					CRF-BP	GP				NULL	dopamine neurons	NULL	NULL	NULL	NULL	gw60_neuron_39_3_401_s_116	12895416	(F) When CRF is bound to CRF-BP it can activate CRF-R2 and the PLC pathway to potentiate NMDARs in dopamine neurons.	bind
15101	2	5444	6	10	NULL	NULL	NULL	CRF	GP		activate					CRF-R2	GP				NULL	dopamine neurons	NULL	NULL	NULL	NULL	gw60_neuron_39_3_401_s_116	12895416	(F) When CRF is bound to CRF-BP it can activate CRF-R2 and the PLC pathway to potentiate NMDARs in dopamine neurons.	bind
15102	3	5444	6	10	NULL	NULL	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_39_3_401_s_116	12895416	(F) When CRF is bound to CRF-BP it can activate CRF-R2 and the PLC pathway to potentiate NMDARs in dopamine neurons.	bind
15226	4	5444	6	10	NULL	NULL	NULL	CRF	GP		activate					PLC pathway	Process				NULL	dopamine neurons	NULL	NULL	NULL	NULL	gw60_neuron_39_3_401_s_116	12895416	(F) When CRF is bound to CRF-BP it can activate CRF-R2 and the PLC pathway to potentiate NMDARs in dopamine neurons.	bind
15227	5	5444	6	10	NULL	NULL	NULL	statement 1	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_39_3_401_s_116	12895416	(F) When CRF is bound to CRF-BP it can activate CRF-R2 and the PLC pathway to potentiate NMDARs in dopamine neurons.	bind
15228	6	5444	6	10	NULL	NULL	NULL	CRF	GP		potentiate					NMDARs	GP				NULL	dopamine neurons	NULL	NULL	NULL	NULL	gw60_neuron_39_3_401_s_116	12895416	(F) When CRF is bound to CRF-BP it can activate CRF-R2 and the PLC pathway to potentiate NMDARs in dopamine neurons.	bind
15229	7	5444	6	10	NULL	NULL	NULL	statement 4	Process		leads to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_39_3_401_s_116	12895416	(F) When CRF is bound to CRF-BP it can activate CRF-R2 and the PLC pathway to potentiate NMDARs in dopamine neurons.	bind
15492	1	5444	7	10	NULL	NULL	NULL	CRF	GP		binds					CRF-BP	GP				NULL	dopamine neurons	NULL	NULL	NULL	NULL	gw60_neuron_39_3_401_s_116	12895416	(F) When CRF is bound to CRF-BP it can activate CRF-R2 and the PLC pathway to potentiate NMDARs in dopamine neurons.	bind
15493	2	5444	7	10	NULL	NULL	NULL	statement 1	Process		activates					CRF-R2	GP				NULL	dopamine neurons	NULL	NULL	NULL	NULL	gw60_neuron_39_3_401_s_116	12895416	(F) When CRF is bound to CRF-BP it can activate CRF-R2 and the PLC pathway to potentiate NMDARs in dopamine neurons.	bind
15494	3	5444	7	10	NULL	NULL	NULL	statement 1	Process		activates					PLC pathway	Process				NULL	dopamine neurons	NULL	NULL	NULL	NULL	gw60_neuron_39_3_401_s_116	12895416	(F) When CRF is bound to CRF-BP it can activate CRF-R2 and the PLC pathway to potentiate NMDARs in dopamine neurons.	bind
15495	4	5444	7	10	NULL	NULL	NULL	statement 2	Process		potentiate					NMDARs	GP				NULL	dopamine neurons	NULL	NULL	NULL	NULL	gw60_neuron_39_3_401_s_116	12895416	(F) When CRF is bound to CRF-BP it can activate CRF-R2 and the PLC pathway to potentiate NMDARs in dopamine neurons.	bind
15496	5	5444	7	10	NULL	NULL	NULL	statement 3	Process		potentiate					NMDARs	GP				NULL	dopamine neurons	NULL	NULL	NULL	NULL	gw60_neuron_39_3_401_s_116	12895416	(F) When CRF is bound to CRF-BP it can activate CRF-R2 and the PLC pathway to potentiate NMDARs in dopamine neurons.	bind
15103	1	5445	6	10	NULL	NULL	NULL	F5CG	GP		bind					DNMT1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_46_33011_s_244	10551869	(F/MeCG)12 has two characteristics as follows: on the one hand, it acts as a dead-end inhibitor since F5CG binds to DNMT1 in the presence of AdoMet and traps the enzyme into a stable DNMT1-AdoMet-DNA complex that does not proceed through catalysis ( 52-54).	bind
15104	2	5445	6	10	NULL	NULL	NULL	statement 1	Process		occurs in presence of					AdoMet	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_46_33011_s_244	10551869	(F/MeCG)12 has two characteristics as follows: on the one hand, it acts as a dead-end inhibitor since F5CG binds to DNMT1 in the presence of AdoMet and traps the enzyme into a stable DNMT1-AdoMet-DNA complex that does not proceed through catalysis ( 52-54).	bind
15231	3	5445	6	10	NULL	NULL	NULL	(F/MeCG)12	Chemical		acts as a					inhibitor	Chemical	dead-end			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_46_33011_s_244	10551869	(F/MeCG)12 has two characteristics as follows: on the one hand, it acts as a dead-end inhibitor since F5CG binds to DNMT1 in the presence of AdoMet and traps the enzyme into a stable DNMT1-AdoMet-DNA complex that does not proceed through catalysis ( 52-54).	bind
15232	4	5445	6	10	NULL	NULL	NULL	statement 2	Process		forms a					DNMT1-AdoMet-DNA complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_46_33011_s_244	10551869	(F/MeCG)12 has two characteristics as follows: on the one hand, it acts as a dead-end inhibitor since F5CG binds to DNMT1 in the presence of AdoMet and traps the enzyme into a stable DNMT1-AdoMet-DNA complex that does not proceed through catalysis ( 52-54).	bind
53093	5	5445	6	10	NULL	NULL	NULL	statement 4	Process		does not proceed through					catalysis	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_46_33011_s_244	10551869	(F/MeCG)12 has two characteristics as follows: on the one hand, it acts as a dead-end inhibitor since F5CG binds to DNMT1 in the presence of AdoMet and traps the enzyme into a stable DNMT1-AdoMet-DNA complex that does not proceed through catalysis ( 52-54).	bind
15497	1	5445	7	10	NULL	NULL	NULL	F5CG	GP		binds to					DNMT1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_46_33011_s_244	10551869	(F/MeCG)12 has two characteristics as follows: on the one hand, it acts as a dead-end inhibitor since F5CG binds to DNMT1 in the presence of AdoMet and traps the enzyme into a stable DNMT1-AdoMet-DNA complex that does not proceed through catalysis ( 52-54).	bind
15498	3	5445	7	10	NULL	NULL	NULL	statement 1	Process		forms					DNMT1-AdoMet-DNA complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_46_33011_s_244	10551869	(F/MeCG)12 has two characteristics as follows: on the one hand, it acts as a dead-end inhibitor since F5CG binds to DNMT1 in the presence of AdoMet and traps the enzyme into a stable DNMT1-AdoMet-DNA complex that does not proceed through catalysis ( 52-54).	bind
15499	4	5445	7	10	NULL	NULL	NULL	statement 3	Process		does not proceed through					catalysis	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_46_33011_s_244	10551869	(F/MeCG)12 has two characteristics as follows: on the one hand, it acts as a dead-end inhibitor since F5CG binds to DNMT1 in the presence of AdoMet and traps the enzyme into a stable DNMT1-AdoMet-DNA complex that does not proceed through catalysis ( 52-54).	bind
20002	2	5445	7	10	NULL	NULL	NULL	statement 1	Process		occurs in the presence of					AdoMet	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_46_33011_s_244	10551869	(F/MeCG)12 has two characteristics as follows: on the one hand, it acts as a dead-end inhibitor since F5CG binds to DNMT1 in the presence of AdoMet and traps the enzyme into a stable DNMT1-AdoMet-DNA complex that does not proceed through catalysis ( 52-54).	bind
15105	1	5446	6	10	NULL	NULL	NULL	Fas-associated factor 1	GP		bind					Fas	GP				NULL		NULL	NULL	NULL	NULL	gw70_nature_425_6959_727_s_69	14562105	(Fas-associated factor 1), a protein  that binds to Fas and regulates apoptosis 5,  6.	bind
15106	2	5446	6	10	NULL	NULL	NULL	Fas-associated factor 1	GP		regulates					apoptosis 5,6	Process				NULL		NULL	NULL	NULL	NULL	gw70_nature_425_6959_727_s_69	14562105	(Fas-associated factor 1), a protein  that binds to Fas and regulates apoptosis 5,  6.	bind
15500	1	5446	7	10	NULL	NULL	NULL	Fas-associated factor 1	GP		binds					Fas	GP				NULL		NULL	NULL	NULL	NULL	gw70_nature_425_6959_727_s_69	14562105	(Fas-associated factor 1), a protein  that binds to Fas and regulates apoptosis 5,  6.	bind
15501	2	5446	7	10	NULL	NULL	NULL	statement 1	Process		regulates					apoptosis5,6	Process				NULL		NULL	NULL	NULL	NULL	gw70_nature_425_6959_727_s_69	14562105	(Fas-associated factor 1), a protein  that binds to Fas and regulates apoptosis 5,  6.	bind
15107	1	5447	6	10	NULL	NULL	NULL	(Fe3+ citrate)2	Chemical		bind					FecA	GP	outer membrane protein			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_7_2387_s_7	12644513	(Fe3+ citrate)2 binds to the outer membrane protein FecA and without further transport into the cell induces transcription of the  fec transport genes ( ,  ).	bind
15194	2	5447	6	10	NULL	NULL	NULL	statement 1	Process		induces					fec transport genes	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_7_2387_s_7	12644513	(Fe3+ citrate)2 binds to the outer membrane protein FecA and without further transport into the cell induces transcription of the  fec transport genes ( ,  ).	bind
44764	3	5447	6	10	NULL	NULL	NULL	(Fe3+ citrate)2	Chemical		is transported into					cell	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_7_2387_s_7	12644513	(Fe3+ citrate)2 binds to the outer membrane protein FecA and without further transport into the cell induces transcription of the  fec transport genes ( ,  ).	bind
44765	4	5447	6	10	NULL	NULL	NULL	statement 2	Process		occurs without					statement 3	Process	further			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_7_2387_s_7	12644513	(Fe3+ citrate)2 binds to the outer membrane protein FecA and without further transport into the cell induces transcription of the  fec transport genes ( ,  ).	bind
15502	1	5447	7	10	NULL	NULL	NULL	(Fe3+ citrate)2	Chemical		binds					FecA	GP	outer membrane protein			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_7_2387_s_7	12644513	(Fe3+ citrate)2 binds to the outer membrane protein FecA and without further transport into the cell induces transcription of the  fec transport genes ( ,  ).	bind
15503	2	5447	7	10	NULL	NULL	NULL	statement 1	Process		induces					fec transport gene	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_7_2387_s_7	12644513	(Fe3+ citrate)2 binds to the outer membrane protein FecA and without further transport into the cell induces transcription of the  fec transport genes ( ,  ).	bind
44762	3	5447	7	10	NULL	NULL	NULL	(Fe3+ citrate)2	Chemical		is transported into					cell	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_7_2387_s_7	12644513	(Fe3+ citrate)2 binds to the outer membrane protein FecA and without further transport into the cell induces transcription of the  fec transport genes ( ,  ).	bind
44763	4	5447	7	10	NULL	NULL	NULL	statement 2	Process		occurs without					statement 3	Process	further			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_7_2387_s_7	12644513	(Fe3+ citrate)2 binds to the outer membrane protein FecA and without further transport into the cell induces transcription of the  fec transport genes ( ,  ).	bind
15195	1	5450	6	10	NULL	NULL	NULL	p-toluic acid	Chemical		bind					AcmACP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_18_12508_s_263	10212227	(Fig.  6,  lanes 2 and  2'') This findings clearly show that the  p-toluic acid bound to AcmACP directly acylates the threonine covalently bound to ACMS II.	bind
15196	2	5450	6	10	NULL	NULL	NULL	threonine	AminoAcid		bind		covalently			ACMS II	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_18_12508_s_263	10212227	(Fig.  6,  lanes 2 and  2'') This findings clearly show that the  p-toluic acid bound to AcmACP directly acylates the threonine covalently bound to ACMS II.	bind
15197	3	5450	6	10	NULL	NULL	NULL	statement 1	Process		acylates		directly			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_18_12508_s_263	10212227	(Fig.  6,  lanes 2 and  2'') This findings clearly show that the  p-toluic acid bound to AcmACP directly acylates the threonine covalently bound to ACMS II.	bind
15504	1	5450	7	10	NULL	NULL	NULL	p-toluic acid	Chemical		bind					AcmACP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_18_12508_s_263	10212227	(Fig.  6,  lanes 2 and  2'') This findings clearly show that the  p-toluic acid bound to AcmACP directly acylates the threonine covalently bound to ACMS II.	bind
15505	2	5450	7	10	NULL	NULL	NULL	threonine	AminoAcid		bind		covalently			ACMS II	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_18_12508_s_263	10212227	(Fig.  6,  lanes 2 and  2'') This findings clearly show that the  p-toluic acid bound to AcmACP directly acylates the threonine covalently bound to ACMS II.	bind
15506	3	5450	7	10	NULL	NULL	NULL	statement 1	Process		acylates		directly			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_18_12508_s_263	10212227	(Fig.  6,  lanes 2 and  2'') This findings clearly show that the  p-toluic acid bound to AcmACP directly acylates the threonine covalently bound to ACMS II.	bind
15198	1	5452	6	10	NULL	NULL	NULL	AtVTI1a	GP		does not bind					T7 antibody	GP				NULL	wild-type plant extract	NULL	NULL	NULL	NULL	gw60_molbiolcell_10_7_2251_s_376	10397763	(Figure  10, right side) As we expected, in the control experiment in which wild-type plant extract was used (Figure  10, left side), AtVTI1a did not bind to the T7 antibody.	bind
15507	1	5452	7	10	NULL	NULL	NULL	AtVTI1a	GP		does not bind					T7 antibody	GP				NULL	wild-type plant extract	NULL	NULL	NULL	NULL	gw60_molbiolcell_10_7_2251_s_376	10397763	(Figure  10, right side) As we expected, in the control experiment in which wild-type plant extract was used (Figure  10, left side), AtVTI1a did not bind to the T7 antibody.	bind
15199	1	5453	6	10	NULL	NULL	NULL	p65	GP		bind					NF-kappaB	GP			consensus sequence	NULL	Nucleus	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1148_s_204	15802625	(Figure II) but increases p65 phosphorylation and p65 binding to NF-kappaB consensus sequence in the nuclei ( Figure 3A and 3B)	bind
15508	1	5453	7	10	NULL	NULL	NULL	p65 	GP		bind					NF-kappaB	GP			consensus sequence	NULL	nucleus	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1148_s_204	15802625	(Figure II) but increases p65 phosphorylation and p65 binding to NF-kappaB consensus sequence in the nuclei ( Figure 3A and 3B)	bind
15200	1	5454	6	10	NULL	NULL	NULL	QKI	GP		regulates					mRNA homeostasis	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_8_1801_s_213	12682013	(Figures  1 and  2), the modulation of the RNA-binding activity of QKI by Src-PTKs (Figures  5 and  6) and the developmental regulation of QKI tyrosine phosphorylation (Figure  8) support the hypothesis that QKI is a pivotal intermediate for developmental signals to control CNS myelination via regulating mRNA homeostasis.	bind
15201	2	5454	6	10	NULL	NULL	NULL	QKI	GP		controls					CNS	OrganismPart	myelination of 			NULL		NULL	NULL	NULL	NULL	gw60_embo_22_8_1801_s_213	12682013	(Figures  1 and  2), the modulation of the RNA-binding activity of QKI by Src-PTKs (Figures  5 and  6) and the developmental regulation of QKI tyrosine phosphorylation (Figure  8) support the hypothesis that QKI is a pivotal intermediate for developmental signals to control CNS myelination via regulating mRNA homeostasis.	bind
15202	3	5454	6	10	NULL	NULL	NULL	statement 2	Process		occurs via					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_8_1801_s_213	12682013	(Figures  1 and  2), the modulation of the RNA-binding activity of QKI by Src-PTKs (Figures  5 and  6) and the developmental regulation of QKI tyrosine phosphorylation (Figure  8) support the hypothesis that QKI is a pivotal intermediate for developmental signals to control CNS myelination via regulating mRNA homeostasis.	bind
53094	4	5454	6	10	NULL	NULL	NULL	QKI	GP		bind					RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_8_1801_s_213	12682013	(Figures  1 and  2), the modulation of the RNA-binding activity of QKI by Src-PTKs (Figures  5 and  6) and the developmental regulation of QKI tyrosine phosphorylation (Figure  8) support the hypothesis that QKI is a pivotal intermediate for developmental signals to control CNS myelination via regulating mRNA homeostasis.	bind
53095	5	5454	6	10	NULL	NULL	NULL	Src-PTKs	GP		modulate					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_8_1801_s_213	12682013	(Figures  1 and  2), the modulation of the RNA-binding activity of QKI by Src-PTKs (Figures  5 and  6) and the developmental regulation of QKI tyrosine phosphorylation (Figure  8) support the hypothesis that QKI is a pivotal intermediate for developmental signals to control CNS myelination via regulating mRNA homeostasis.	bind
53096	6	5454	6	10	NULL	NULL	NULL	QKI	GP		acts as					pivotal intermediate	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_8_1801_s_213	12682013	(Figures  1 and  2), the modulation of the RNA-binding activity of QKI by Src-PTKs (Figures  5 and  6) and the developmental regulation of QKI tyrosine phosphorylation (Figure  8) support the hypothesis that QKI is a pivotal intermediate for developmental signals to control CNS myelination via regulating mRNA homeostasis.	bind
15509	1	5454	7	10	NULL	NULL	NULL	QKI	GP		bind					RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_8_1801_s_213	12682013	(Figures  1 and  2), the modulation of the RNA-binding activity of QKI by Src-PTKs (Figures  5 and  6) and the developmental regulation of QKI tyrosine phosphorylation (Figure  8) support the hypothesis that QKI is a pivotal intermediate for developmental signals to control CNS myelination via regulating mRNA homeostasis.	bind
15510	2	5454	7	10	NULL	NULL	NULL	Src-PTKs	GP		modulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_8_1801_s_213	12682013	(Figures  1 and  2), the modulation of the RNA-binding activity of QKI by Src-PTKs (Figures  5 and  6) and the developmental regulation of QKI tyrosine phosphorylation (Figure  8) support the hypothesis that QKI is a pivotal intermediate for developmental signals to control CNS myelination via regulating mRNA homeostasis.	bind
53097	3	5454	7	10	NULL	NULL	NULL	QKI	GP		regulates					mRNA homeostasis	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_8_1801_s_213	12682013	(Figures  1 and  2), the modulation of the RNA-binding activity of QKI by Src-PTKs (Figures  5 and  6) and the developmental regulation of QKI tyrosine phosphorylation (Figure  8) support the hypothesis that QKI is a pivotal intermediate for developmental signals to control CNS myelination via regulating mRNA homeostasis.	bind
53098	4	5454	7	10	NULL	NULL	NULL	QKI	GP		controls					CNS	OrganismPart	myelination of 			NULL		NULL	NULL	NULL	NULL	gw60_embo_22_8_1801_s_213	12682013	(Figures  1 and  2), the modulation of the RNA-binding activity of QKI by Src-PTKs (Figures  5 and  6) and the developmental regulation of QKI tyrosine phosphorylation (Figure  8) support the hypothesis that QKI is a pivotal intermediate for developmental signals to control CNS myelination via regulating mRNA homeostasis.	bind
53099	5	5454	7	10	NULL	NULL	NULL	statement 4	Process		via					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_8_1801_s_213	12682013	(Figures  1 and  2), the modulation of the RNA-binding activity of QKI by Src-PTKs (Figures  5 and  6) and the developmental regulation of QKI tyrosine phosphorylation (Figure  8) support the hypothesis that QKI is a pivotal intermediate for developmental signals to control CNS myelination via regulating mRNA homeostasis.	bind
53100	6	5454	7	10	NULL	NULL	NULL	QKI	GP		acts as					pivotal intermediate	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_8_1801_s_213	12682013	(Figures  1 and  2), the modulation of the RNA-binding activity of QKI by Src-PTKs (Figures  5 and  6) and the developmental regulation of QKI tyrosine phosphorylation (Figure  8) support the hypothesis that QKI is a pivotal intermediate for developmental signals to control CNS myelination via regulating mRNA homeostasis.	bind
15203	1	5455	6	10	NULL	NULL	NULL	MCAK	GP		bind					MT lattice	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_2_700_s_182	16291860	(Figures  1 and  4); therefore, the high-affinity end binding sites for MCAK on the MT are saturated, and MCAK is binding to the MT lattice as well.	bind
15514	1	5455	7	10	NULL	NULL	NULL	MCAK	GP		binds					MT lattice	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_2_700_s_182	16291860	(Figures  1 and  4); therefore, the high-affinity end binding sites for MCAK on the MT are saturated, and MCAK is binding to the MT lattice as well.	bind
15204	1	5457	6	10	NULL	NULL	NULL	p70	GP		bind					splicosomal complex	CellComponent	mature	3 splice site		NULL		NULL	NULL	NULL	NULL	gw60_embo_16_14_4421_s_118	9250686	(Figures  2 and  3A); the kinetics of p70 crosslinking parallel those of the second step of splicing (Figures  1B); both the second step of splicing and crosslinking of p70 require a normal RNA branch structure (Figure  4); p70 is bound to the 3  splice site in the mature spliceosomal complex (Figure  3); certain  cis-acting mutations impair both the binding of p70 and the second step of splicing	bind
15208	2	5457	6	10	NULL	NULL	NULL	cis-acting mutations	Process		impair					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_14_4421_s_118	9250686	(Figures  2 and  3A); the kinetics of p70 crosslinking parallel those of the second step of splicing (Figures  1B); both the second step of splicing and crosslinking of p70 require a normal RNA branch structure (Figure  4); p70 is bound to the 3  splice site in the mature spliceosomal complex (Figure  3); certain  cis-acting mutations impair both the binding of p70 and the second step of splicing	bind
19043	3	5457	6	10	NULL	NULL	NULL	second step of splicing	Process		require					RNA branch structure	NucleicAcid	normal			NULL		NULL	NULL	NULL	NULL	gw60_embo_16_14_4421_s_118	9250686	(Figures  2 and  3A); the kinetics of p70 crosslinking parallel those of the second step of splicing (Figures  1B); both the second step of splicing and crosslinking of p70 require a normal RNA branch structure (Figure  4); p70 is bound to the 3  splice site in the mature spliceosomal complex (Figure  3); certain  cis-acting mutations impair both the binding of p70 and the second step of splicing	bind
19044	4	5457	6	10	NULL	NULL	NULL	p70	GP	crosslinking of	require					RNA branch structure	NucleicAcid	normal			NULL		NULL	NULL	NULL	NULL	gw60_embo_16_14_4421_s_118	9250686	(Figures  2 and  3A); the kinetics of p70 crosslinking parallel those of the second step of splicing (Figures  1B); both the second step of splicing and crosslinking of p70 require a normal RNA branch structure (Figure  4); p70 is bound to the 3  splice site in the mature spliceosomal complex (Figure  3); certain  cis-acting mutations impair both the binding of p70 and the second step of splicing	bind
19045	5	5457	6	10	NULL	NULL	NULL	cis acting mutations	Process		impair					second step of splicing	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_14_4421_s_118	9250686	(Figures  2 and  3A); the kinetics of p70 crosslinking parallel those of the second step of splicing (Figures  1B); both the second step of splicing and crosslinking of p70 require a normal RNA branch structure (Figure  4); p70 is bound to the 3  splice site in the mature spliceosomal complex (Figure  3); certain  cis-acting mutations impair both the binding of p70 and the second step of splicing	bind
15515	1	5457	7	10	NULL	NULL	NULL	second step of splicing	Process		require					RNA branch structure	NucleicAcid	normal			NULL		NULL	NULL	NULL	NULL	gw60_embo_16_14_4421_s_118	9250686	(Figures  2 and  3A); the kinetics of p70 crosslinking parallel those of the second step of splicing (Figures  1B); both the second step of splicing and crosslinking of p70 require a normal RNA branch structure (Figure  4); p70 is bound to the 3  splice site in the mature spliceosomal complex (Figure  3); certain  cis-acting mutations impair both the binding of p70 and the second step of splicing	bind
15516	2	5457	7	10	NULL	NULL	NULL	p70	GP	crosslinking of	requires					RNA branch structure	NucleicAcid	normal			NULL		NULL	NULL	NULL	NULL	gw60_embo_16_14_4421_s_118	9250686	(Figures  2 and  3A); the kinetics of p70 crosslinking parallel those of the second step of splicing (Figures  1B); both the second step of splicing and crosslinking of p70 require a normal RNA branch structure (Figure  4); p70 is bound to the 3  splice site in the mature spliceosomal complex (Figure  3); certain  cis-acting mutations impair both the binding of p70 and the second step of splicing	bind
15517	3	5457	7	10	NULL	NULL	NULL	p70	GP		binds					spliceosomal complex	CellComponent	mature	3 splice site		NULL		NULL	NULL	NULL	NULL	gw60_embo_16_14_4421_s_118	9250686	(Figures  2 and  3A); the kinetics of p70 crosslinking parallel those of the second step of splicing (Figures  1B); both the second step of splicing and crosslinking of p70 require a normal RNA branch structure (Figure  4); p70 is bound to the 3  splice site in the mature spliceosomal complex (Figure  3); certain  cis-acting mutations impair both the binding of p70 and the second step of splicing	bind
15518	4	5457	7	10	NULL	NULL	NULL	cis-acting mutations	Process		impair					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_14_4421_s_118	9250686	(Figures  2 and  3A); the kinetics of p70 crosslinking parallel those of the second step of splicing (Figures  1B); both the second step of splicing and crosslinking of p70 require a normal RNA branch structure (Figure  4); p70 is bound to the 3  splice site in the mature spliceosomal complex (Figure  3); certain  cis-acting mutations impair both the binding of p70 and the second step of splicing	bind
15519	5	5457	7	10	NULL	NULL	NULL	cis-acting mutations	Process		impair					second step of splicing	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_14_4421_s_118	9250686	(Figures  2 and  3A); the kinetics of p70 crosslinking parallel those of the second step of splicing (Figures  1B); both the second step of splicing and crosslinking of p70 require a normal RNA branch structure (Figure  4); p70 is bound to the 3  splice site in the mature spliceosomal complex (Figure  3); certain  cis-acting mutations impair both the binding of p70 and the second step of splicing	bind
15209	1	5459	6	10	NULL	NULL	NULL	IgE antibodies	GP		did not bind					HSA	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_293_5_1348_s_92	12054661	(First of all, from this study, we could confirm that patients'' IgE antibodies did not bind to HSA which was used in "`blocking"` step.)	bind
15520	1	5459	7	10	NULL	NULL	NULL	IgE antibodies	GP		does not bind					HSA	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_293_5_1348_s_92	12054661	(First of all, from this study, we could confirm that patients'' IgE antibodies did not bind to HSA which was used in "`blocking"` step.)	bind
15210	1	5460	6	10	NULL	NULL	NULL	KDR	GP		is					kinase insert domain-containing receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_6_3154_s_40	8621715	(Fms-like tyrosine kinase) ( 24) and KDR  (kinase insert domain-containing receptor) proteins ( 25,  26) (the mouse homologue of the latter is called  Flk-1; see ( 27) ), bind VEGF with high affinity.	bind
15211	2	5460	6	10	NULL	NULL	NULL	KDR	GP		bind		high affinity			VEGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_6_3154_s_40	8621715	(Fms-like tyrosine kinase) ( 24) and KDR  (kinase insert domain-containing receptor) proteins ( 25,  26) (the mouse homologue of the latter is called  Flk-1; see ( 27) ), bind VEGF with high affinity.	bind
15212	3	5460	6	10	NULL	NULL	NULL	Flk-1	GP	mouse	is homologous to					KDR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_6_3154_s_40	8621715	(Fms-like tyrosine kinase) ( 24) and KDR  (kinase insert domain-containing receptor) proteins ( 25,  26) (the mouse homologue of the latter is called  Flk-1; see ( 27) ), bind VEGF with high affinity.	bind
15522	1	5460	7	10	NULL	NULL	NULL	KDR	GP		bind		high affinity			VEGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_6_3154_s_40	8621715	(Fms-like tyrosine kinase) ( 24) and KDR  (kinase insert domain-containing receptor) proteins ( 25,  26) (the mouse homologue of the latter is called  Flk-1; see ( 27) ), bind VEGF with high affinity.	bind
15524	2	5460	7	10	NULL	NULL	NULL	KDR	GP		is					kinase insert domain-containing receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_6_3154_s_40	8621715	(Fms-like tyrosine kinase) ( 24) and KDR  (kinase insert domain-containing receptor) proteins ( 25,  26) (the mouse homologue of the latter is called  Flk-1; see ( 27) ), bind VEGF with high affinity.	bind
19607	3	5460	7	10	NULL	NULL	NULL	Flk-1	GP	mouse	is homologous to					KDR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_6_3154_s_40	8621715	(Fms-like tyrosine kinase) ( 24) and KDR  (kinase insert domain-containing receptor) proteins ( 25,  26) (the mouse homologue of the latter is called  Flk-1; see ( 27) ), bind VEGF with high affinity.	bind
16348	1	5461	6	10	NULL	NULL	NULL	IGFBP-5	GP	human	bind					IGF-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_1_5_655_s_36	11709186	(For example, human IGFBP-5 binds IGF-2 with a dissociation constant of 8 x 10 11 M;  Kalus et al., 1998  ).	bind
15525	1	5461	7	10	NULL	NULL	NULL	IGFBP-5	GP	human	bind					IGF-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_1_5_655_s_36	11709186	(For example, human IGFBP-5 binds IGF-2 with a dissociation constant of 8 x 10 11 M;  Kalus et al., 1998  ).	bind
16349	1	5462	6	10	NULL	NULL	NULL	Ab-p44	GP		bind					TFIIH	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_102_5_599_s_140	11007478	(G and H) Analysis of the binding of Ab-p44 to TFIIH.	bind
15526	1	5462	7	10	NULL	NULL	NULL	 Ab-p44	GP		bind					TFIIH	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_102_5_599_s_140	11007478	(G and H) Analysis of the binding of Ab-p44 to TFIIH.	bind
16350	1	5465	6	10	NULL	NULL	NULL	GTP	Chemical	active	bind					Rac	GP				NULL	lysates of LS174T	NULL	NULL	NULL	NULL	gw60_cell_111_2_251_s_61	12408869	(G) Active GTP-bound Rac was precipitated from lysates of LS174T using PAK1 Rac binding domain coupled to agarose (upper image).	bind
15527	1	5465	7	10	NULL	NULL	NULL	GTP	Chemical	active	bind					Rac	GP				NULL	lysates of LS174T	NULL	NULL	NULL	NULL	gw60_cell_111_2_251_s_61	12408869	(G) Active GTP-bound Rac was precipitated from lysates of LS174T using PAK1 Rac binding domain coupled to agarose (upper image).	bind
16351	1	5466	6	10	NULL	NULL	NULL	Sox2	GP		bind									composite sox-oct element	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_14_6031_s_271	15988017	(G) Analysis of the cooperativity  of Sox2 and Oct4 binding to the composite sox-oct element.	bind
16352	2	5466	6	10	NULL	NULL	NULL	Oct4	GP		bind									composite sox-oct element	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_14_6031_s_271	15988017	(G) Analysis of the cooperativity  of Sox2 and Oct4 binding to the composite sox-oct element.	bind
19046	3	5466	6	10	NULL	NULL	NULL	statement 1	Process		occurs in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_14_6031_s_271	15988017	(G) Analysis of the cooperativity  of Sox2 and Oct4 binding to the composite sox-oct element.	bind
15529	1	5466	7	10	NULL	NULL	NULL	Sox2	GP		bind									composite sox-oct element	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_14_6031_s_271	15988017	(G) Analysis of the cooperativity  of Sox2 and Oct4 binding to the composite sox-oct element.	bind
15530	2	5466	7	10	NULL	NULL	NULL	Oct4	GP		bind									composite sox-oct element	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_14_6031_s_271	15988017	(G) Analysis of the cooperativity  of Sox2 and Oct4 binding to the composite sox-oct element.	bind
15531	3	5466	7	10	NULL	NULL	NULL	statement 1	Process		occurs in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_14_6031_s_271	15988017	(G) Analysis of the cooperativity  of Sox2 and Oct4 binding to the composite sox-oct element.	bind
16353	1	5467	6	10	NULL	NULL	NULL	c-Jun	GP		bind					JNK2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_87_5_929_s_112	8945519	(G) Binding of c-Jun, JunB, or JunD to  JNK2.	bind
16354	2	5467	6	10	NULL	NULL	NULL	JunB	GP		bind					JNK2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_87_5_929_s_112	8945519	(G) Binding of c-Jun, JunB, or JunD to  JNK2.	bind
16355	3	5467	6	10	NULL	NULL	NULL	JunD	GP		bind					JNK2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_87_5_929_s_112	8945519	(G) Binding of c-Jun, JunB, or JunD to  JNK2.	bind
15532	1	5467	7	10	NULL	NULL	NULL	c-Jun	GP		bind					JNK2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_87_5_929_s_112	8945519	(G) Binding of c-Jun, JunB, or JunD to  JNK2.	bind
15533	2	5467	7	10	NULL	NULL	NULL	JunB	GP		bind					JNK2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_87_5_929_s_112	8945519	(G) Binding of c-Jun, JunB, or JunD to  JNK2.	bind
15534	3	5467	7	10	NULL	NULL	NULL	 JunD	GP		bind					JNK2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_87_5_929_s_112	8945519	(G) Binding of c-Jun, JunB, or JunD to  JNK2.	bind
16356	1	5468	6	10	NULL	NULL	NULL	Mnk2a	GP		bind					eIF4G	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_16_5692_s_160	12897141	(G) Binding of Mnk2a to eIF4G enhances eIF4E phosphorylation.	bind
16357	2	5468	6	10	NULL	NULL	NULL	statement 1	Process		enhances					eIF4E	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_16_5692_s_160	12897141	(G) Binding of Mnk2a to eIF4G enhances eIF4E phosphorylation.	bind
15535	1	5468	7	10	NULL	NULL	NULL	Mnk2a	GP		bind					eIF4G	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_16_5692_s_160	12897141	(G) Binding of Mnk2a to eIF4G enhances eIF4E phosphorylation.	bind
15536	2	5468	7	10	NULL	NULL	NULL	statement 1	Process		enhances					eIF4E	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_16_5692_s_160	12897141	(G) Binding of Mnk2a to eIF4G enhances eIF4E phosphorylation.	bind
16365	1	5469	6	10	NULL	NULL	NULL	Cdc31p	GP		bind					hSfi1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_162_7_1211_s_165	14504268	(g) Cdc31p binding to GST fusions of hSfi1.	bind
53101	2	5469	6	10	NULL	NULL	NULL	hSfi1	GP		is a type of					GST fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_162_7_1211_s_165	14504268	(g) Cdc31p binding to GST fusions of hSfi1.	bind
15537	1	5469	7	10	NULL	NULL	NULL	Cdc31p	GP		bind					hSfi1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_162_7_1211_s_165	14504268	(g) Cdc31p binding to GST fusions of hSfi1.	bind
53102	2	5469	7	10	NULL	NULL	NULL	hSfi1	GP		is a type of					GST fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_162_7_1211_s_165	14504268	(g) Cdc31p binding to GST fusions of hSfi1.	bind
16772	1	5470	6	10	NULL	NULL	NULL	noggin RNA	NucleicAcid		increases					BF-1	GP	induction of			NULL		NULL	NULL	NULL	NULL	gw70_development_131_21_5309_s_133	15456729	(G) Co-injection of 2 ng Cv-2 RNA plus 0.1 ng noggin RNA increases the induction  of BF-1 when compared with injection of 0.1 ng noggin RNA alone.	bind
16774	2	5470	6	10	NULL	NULL	NULL	Cv-2 RNA	NucleicAcid		increases					BF-1	GP	induction of			NULL		NULL	NULL	NULL	NULL	gw70_development_131_21_5309_s_133	15456729	(G) Co-injection of 2 ng Cv-2 RNA plus 0.1 ng noggin RNA increases the induction  of BF-1 when compared with injection of 0.1 ng noggin RNA alone.	bind
16775	3	5470	6	10	NULL	NULL	NULL	statement 2	Process		occurs togther with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_131_21_5309_s_133	15456729	(G) Co-injection of 2 ng Cv-2 RNA plus 0.1 ng noggin RNA increases the induction  of BF-1 when compared with injection of 0.1 ng noggin RNA alone.	bind
16777	4	5470	6	10	NULL	NULL	NULL	statement 3	Process		is more as compared with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_131_21_5309_s_133	15456729	(G) Co-injection of 2 ng Cv-2 RNA plus 0.1 ng noggin RNA increases the induction  of BF-1 when compared with injection of 0.1 ng noggin RNA alone.	bind
15538	1	5470	7	10	NULL	NULL	NULL	Cv-2 RNA	NucleicAcid		increase					BF-1	GP	induction of			NULL		NULL	NULL	NULL	NULL	gw70_development_131_21_5309_s_133	15456729	(G) Co-injection of 2 ng Cv-2 RNA plus 0.1 ng noggin RNA increases the induction  of BF-1 when compared with injection of 0.1 ng noggin RNA alone.	bind
15539	2	5470	7	10	NULL	NULL	NULL	noggin RNA	NucleicAcid		increase					BF-1	GP	induction of			NULL		NULL	NULL	NULL	NULL	gw70_development_131_21_5309_s_133	15456729	(G) Co-injection of 2 ng Cv-2 RNA plus 0.1 ng noggin RNA increases the induction  of BF-1 when compared with injection of 0.1 ng noggin RNA alone.	bind
15540	3	5470	7	10	NULL	NULL	NULL	statement 1	Process		occurs togther with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_131_21_5309_s_133	15456729	(G) Co-injection of 2 ng Cv-2 RNA plus 0.1 ng noggin RNA increases the induction  of BF-1 when compared with injection of 0.1 ng noggin RNA alone.	bind
53103	4	5470	7	10	NULL	NULL	NULL	statement 3	Process		is more as compared with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_131_21_5309_s_133	15456729	(G) Co-injection of 2 ng Cv-2 RNA plus 0.1 ng noggin RNA increases the induction  of BF-1 when compared with injection of 0.1 ng noggin RNA alone.	bind
16366	1	5471	6	10	NULL	NULL	NULL	Lz	GP		bind					SME				RD sites 	NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_270	11051549	(G) Cone  cell-specific activation of  D-Pax2 expression is dependent on three inputs: (i) Lz binding to  the RD sites in the eye-specific enhancer (SME), (ii) EGFR signal-dependent inactivation of Yan  and activation of PntP2, which then binds to ETS domain binding sites in  the SME, and (iii) Notch signal-dependent activation of Su(H), which binds to the Su(H) binding sites  in the SME.	bind
16367	2	5471	6	10	NULL	NULL	NULL	SME	GP		is					eye-specific enhancer	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_270	11051549	(G) Cone  cell-specific activation of  D-Pax2 expression is dependent on three inputs: (i) Lz binding to  the RD sites in the eye-specific enhancer (SME), (ii) EGFR signal-dependent inactivation of Yan  and activation of PntP2, which then binds to ETS domain binding sites in  the SME, and (iii) Notch signal-dependent activation of Su(H), which binds to the Su(H) binding sites  in the SME.	bind
16780	3	5471	6	10	NULL	NULL	NULL	EGFR	GP		inactivates					Yan	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_270	11051549	(G) Cone  cell-specific activation of  D-Pax2 expression is dependent on three inputs: (i) Lz binding to  the RD sites in the eye-specific enhancer (SME), (ii) EGFR signal-dependent inactivation of Yan  and activation of PntP2, which then binds to ETS domain binding sites in  the SME, and (iii) Notch signal-dependent activation of Su(H), which binds to the Su(H) binding sites  in the SME.	bind
16782	4	5471	6	10	NULL	NULL	NULL	EGFR	GP		activates					PntP2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_270	11051549	(G) Cone  cell-specific activation of  D-Pax2 expression is dependent on three inputs: (i) Lz binding to  the RD sites in the eye-specific enhancer (SME), (ii) EGFR signal-dependent inactivation of Yan  and activation of PntP2, which then binds to ETS domain binding sites in  the SME, and (iii) Notch signal-dependent activation of Su(H), which binds to the Su(H) binding sites  in the SME.	bind
16820	5	5471	6	10	NULL	NULL	NULL	PntP2	GP		bind					SME	GP			ETS domain binding sites	NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_270	11051549	(G) Cone  cell-specific activation of  D-Pax2 expression is dependent on three inputs: (i) Lz binding to  the RD sites in the eye-specific enhancer (SME), (ii) EGFR signal-dependent inactivation of Yan  and activation of PntP2, which then binds to ETS domain binding sites in  the SME, and (iii) Notch signal-dependent activation of Su(H), which binds to the Su(H) binding sites  in the SME.	bind
16821	6	5471	6	10	NULL	NULL	NULL	Notch signal	Process		activates					Su(H)	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_270	11051549	(G) Cone  cell-specific activation of  D-Pax2 expression is dependent on three inputs: (i) Lz binding to  the RD sites in the eye-specific enhancer (SME), (ii) EGFR signal-dependent inactivation of Yan  and activation of PntP2, which then binds to ETS domain binding sites in  the SME, and (iii) Notch signal-dependent activation of Su(H), which binds to the Su(H) binding sites  in the SME.	bind
16822	7	5471	6	10	NULL	NULL	NULL	Su(H)	GP		bind					SME	GP			Su(H) binding sites	NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_270	11051549	(G) Cone  cell-specific activation of  D-Pax2 expression is dependent on three inputs: (i) Lz binding to  the RD sites in the eye-specific enhancer (SME), (ii) EGFR signal-dependent inactivation of Yan  and activation of PntP2, which then binds to ETS domain binding sites in  the SME, and (iii) Notch signal-dependent activation of Su(H), which binds to the Su(H) binding sites  in the SME.	bind
16823	8	5471	6	10	NULL	NULL	NULL	D-Pax2	GP	expression of	is dependent on					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_270	11051549	(G) Cone  cell-specific activation of  D-Pax2 expression is dependent on three inputs: (i) Lz binding to  the RD sites in the eye-specific enhancer (SME), (ii) EGFR signal-dependent inactivation of Yan  and activation of PntP2, which then binds to ETS domain binding sites in  the SME, and (iii) Notch signal-dependent activation of Su(H), which binds to the Su(H) binding sites  in the SME.	bind
16826	9	5471	6	10	NULL	NULL	NULL	D-Pax2	GP	expression of	is dependent on					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_270	11051549	(G) Cone  cell-specific activation of  D-Pax2 expression is dependent on three inputs: (i) Lz binding to  the RD sites in the eye-specific enhancer (SME), (ii) EGFR signal-dependent inactivation of Yan  and activation of PntP2, which then binds to ETS domain binding sites in  the SME, and (iii) Notch signal-dependent activation of Su(H), which binds to the Su(H) binding sites  in the SME.	bind
16827	10	5471	6	10	NULL	NULL	NULL	D-Pax2	GP	expression of	is dependent on					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_270	11051549	(G) Cone  cell-specific activation of  D-Pax2 expression is dependent on three inputs: (i) Lz binding to  the RD sites in the eye-specific enhancer (SME), (ii) EGFR signal-dependent inactivation of Yan  and activation of PntP2, which then binds to ETS domain binding sites in  the SME, and (iii) Notch signal-dependent activation of Su(H), which binds to the Su(H) binding sites  in the SME.	bind
16831	11	5471	6	10	NULL	NULL	NULL	D-Pax2	GP	expression of	is dependent on					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_270	11051549	(G) Cone  cell-specific activation of  D-Pax2 expression is dependent on three inputs: (i) Lz binding to  the RD sites in the eye-specific enhancer (SME), (ii) EGFR signal-dependent inactivation of Yan  and activation of PntP2, which then binds to ETS domain binding sites in  the SME, and (iii) Notch signal-dependent activation of Su(H), which binds to the Su(H) binding sites  in the SME.	bind
16832	12	5471	6	10	NULL	NULL	NULL	D-Pax2	GP	expression of	is dependent on					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_270	11051549	(G) Cone  cell-specific activation of  D-Pax2 expression is dependent on three inputs: (i) Lz binding to  the RD sites in the eye-specific enhancer (SME), (ii) EGFR signal-dependent inactivation of Yan  and activation of PntP2, which then binds to ETS domain binding sites in  the SME, and (iii) Notch signal-dependent activation of Su(H), which binds to the Su(H) binding sites  in the SME.	bind
16834	13	5471	6	10	NULL	NULL	NULL	D-Pax2	GP	expression of	is dependent on					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_270	11051549	(G) Cone  cell-specific activation of  D-Pax2 expression is dependent on three inputs: (i) Lz binding to  the RD sites in the eye-specific enhancer (SME), (ii) EGFR signal-dependent inactivation of Yan  and activation of PntP2, which then binds to ETS domain binding sites in  the SME, and (iii) Notch signal-dependent activation of Su(H), which binds to the Su(H) binding sites  in the SME.	bind
15541	1	5471	7	10	NULL	NULL	NULL	Lz	GP		bind					SME	GP			RD sites 	NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_270	11051549	(G) Cone  cell-specific activation of  D-Pax2 expression is dependent on three inputs: (i) Lz binding to  the RD sites in the eye-specific enhancer (SME), (ii) EGFR signal-dependent inactivation of Yan  and activation of PntP2, which then binds to ETS domain binding sites in  the SME, and (iii) Notch signal-dependent activation of Su(H), which binds to the Su(H) binding sites  in the SME.	bind
15542	2	5471	7	10	NULL	NULL	NULL	EGFR	GP		inactivate					Yan	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_270	11051549	(G) Cone  cell-specific activation of  D-Pax2 expression is dependent on three inputs: (i) Lz binding to  the RD sites in the eye-specific enhancer (SME), (ii) EGFR signal-dependent inactivation of Yan  and activation of PntP2, which then binds to ETS domain binding sites in  the SME, and (iii) Notch signal-dependent activation of Su(H), which binds to the Su(H) binding sites  in the SME.	bind
15543	3	5471	7	10	NULL	NULL	NULL	EGFR	GP		activates					PntP2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_270	11051549	(G) Cone  cell-specific activation of  D-Pax2 expression is dependent on three inputs: (i) Lz binding to  the RD sites in the eye-specific enhancer (SME), (ii) EGFR signal-dependent inactivation of Yan  and activation of PntP2, which then binds to ETS domain binding sites in  the SME, and (iii) Notch signal-dependent activation of Su(H), which binds to the Su(H) binding sites  in the SME.	bind
15544	4	5471	7	10	NULL	NULL	NULL	statement 3	Process		binds to					SME	GP			ETS domain binding site	NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_270	11051549	(G) Cone  cell-specific activation of  D-Pax2 expression is dependent on three inputs: (i) Lz binding to  the RD sites in the eye-specific enhancer (SME), (ii) EGFR signal-dependent inactivation of Yan  and activation of PntP2, which then binds to ETS domain binding sites in  the SME, and (iii) Notch signal-dependent activation of Su(H), which binds to the Su(H) binding sites  in the SME.	bind
15545	5	5471	7	10	NULL	NULL	NULL	Notch signal	Process		activates					Su(H)	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_270	11051549	(G) Cone  cell-specific activation of  D-Pax2 expression is dependent on three inputs: (i) Lz binding to  the RD sites in the eye-specific enhancer (SME), (ii) EGFR signal-dependent inactivation of Yan  and activation of PntP2, which then binds to ETS domain binding sites in  the SME, and (iii) Notch signal-dependent activation of Su(H), which binds to the Su(H) binding sites  in the SME.	bind
15546	6	5471	7	10	NULL	NULL	NULL	statement 5	Process		bind					SME	GP			Su(H) binding site	NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_270	11051549	(G) Cone  cell-specific activation of  D-Pax2 expression is dependent on three inputs: (i) Lz binding to  the RD sites in the eye-specific enhancer (SME), (ii) EGFR signal-dependent inactivation of Yan  and activation of PntP2, which then binds to ETS domain binding sites in  the SME, and (iii) Notch signal-dependent activation of Su(H), which binds to the Su(H) binding sites  in the SME.	bind
15547	7	5471	7	10	NULL	NULL	NULL	SME	GP		is					eye-specific enhancer	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_270	11051549	(G) Cone  cell-specific activation of  D-Pax2 expression is dependent on three inputs: (i) Lz binding to  the RD sites in the eye-specific enhancer (SME), (ii) EGFR signal-dependent inactivation of Yan  and activation of PntP2, which then binds to ETS domain binding sites in  the SME, and (iii) Notch signal-dependent activation of Su(H), which binds to the Su(H) binding sites  in the SME.	bind
19608	8	5471	7	10	NULL	NULL	NULL	D-Pax2	GP	expression of	is dependent on					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_270	11051549	(G) Cone  cell-specific activation of  D-Pax2 expression is dependent on three inputs: (i) Lz binding to  the RD sites in the eye-specific enhancer (SME), (ii) EGFR signal-dependent inactivation of Yan  and activation of PntP2, which then binds to ETS domain binding sites in  the SME, and (iii) Notch signal-dependent activation of Su(H), which binds to the Su(H) binding sites  in the SME.	bind
19609	9	5471	7	10	NULL	NULL	NULL	D-Pax2	GP	expression of	is dependent on					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_270	11051549	(G) Cone  cell-specific activation of  D-Pax2 expression is dependent on three inputs: (i) Lz binding to  the RD sites in the eye-specific enhancer (SME), (ii) EGFR signal-dependent inactivation of Yan  and activation of PntP2, which then binds to ETS domain binding sites in  the SME, and (iii) Notch signal-dependent activation of Su(H), which binds to the Su(H) binding sites  in the SME.	bind
19610	10	5471	7	10	NULL	NULL	NULL	D-Pax2	GP	expression of	is dependent on 					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_270	11051549	(G) Cone  cell-specific activation of  D-Pax2 expression is dependent on three inputs: (i) Lz binding to  the RD sites in the eye-specific enhancer (SME), (ii) EGFR signal-dependent inactivation of Yan  and activation of PntP2, which then binds to ETS domain binding sites in  the SME, and (iii) Notch signal-dependent activation of Su(H), which binds to the Su(H) binding sites  in the SME.	bind
19611	11	5471	7	10	NULL	NULL	NULL	D-Pax2	GP	expression of	is dependent on					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_270	11051549	(G) Cone  cell-specific activation of  D-Pax2 expression is dependent on three inputs: (i) Lz binding to  the RD sites in the eye-specific enhancer (SME), (ii) EGFR signal-dependent inactivation of Yan  and activation of PntP2, which then binds to ETS domain binding sites in  the SME, and (iii) Notch signal-dependent activation of Su(H), which binds to the Su(H) binding sites  in the SME.	bind
19612	12	5471	7	10	NULL	NULL	NULL	D-Pax2	GP	expression of	is dependent on					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_270	11051549	(G) Cone  cell-specific activation of  D-Pax2 expression is dependent on three inputs: (i) Lz binding to  the RD sites in the eye-specific enhancer (SME), (ii) EGFR signal-dependent inactivation of Yan  and activation of PntP2, which then binds to ETS domain binding sites in  the SME, and (iii) Notch signal-dependent activation of Su(H), which binds to the Su(H) binding sites  in the SME.	bind
19613	13	5471	7	10	NULL	NULL	NULL	D-Pax2	GP	expression of	is dependent on					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_270	11051549	(G) Cone  cell-specific activation of  D-Pax2 expression is dependent on three inputs: (i) Lz binding to  the RD sites in the eye-specific enhancer (SME), (ii) EGFR signal-dependent inactivation of Yan  and activation of PntP2, which then binds to ETS domain binding sites in  the SME, and (iii) Notch signal-dependent activation of Su(H), which binds to the Su(H) binding sites  in the SME.	bind
16369	1	5472	6	10	NULL	NULL	NULL	SRF	GP	epitope tagged	bind							radioactively labeled		SRE	NULL		NULL	NULL	NULL	NULL	gw60_cell_110_6_713_s_242	12297045	(G) EMSA reveals binding of epitope tagged SRF to radioactively labeled SRE (lanes 1,3).	bind
15548	1	5472	7	10	NULL	NULL	NULL	SRF	GP	epitope tagged	bind							radioactively labeled		SRE	NULL		NULL	NULL	NULL	NULL	gw60_cell_110_6_713_s_242	12297045	(G) EMSA reveals binding of epitope tagged SRF to radioactively labeled SRE (lanes 1,3).	bind
16370	1	5473	6	10	NULL	NULL	NULL	Tem1	GP		bind					Bub2	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_219_s_271	14734533	(G) Gic1-pr and Gic1-pr-SS disrupt the binding  between Tem1 and Bub2 in vitro.	bind
16371	2	5473	6	10	NULL	NULL	NULL	Gic1-pr	GP		disrupts					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_219_s_271	14734533	(G) Gic1-pr and Gic1-pr-SS disrupt the binding  between Tem1 and Bub2 in vitro.	bind
16372	3	5473	6	10	NULL	NULL	NULL	Gic1-pr-SS	GP		disrupts					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_219_s_271	14734533	(G) Gic1-pr and Gic1-pr-SS disrupt the binding  between Tem1 and Bub2 in vitro.	bind
15549	1	5473	7	10	NULL	NULL	NULL	Tem1	GP		bind					Bub2	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_219_s_271	14734533	(G) Gic1-pr and Gic1-pr-SS disrupt the binding  between Tem1 and Bub2 in vitro.	bind
15550	2	5473	7	10	NULL	NULL	NULL	Gic1-pr	GP		disrupts					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_219_s_271	14734533	(G) Gic1-pr and Gic1-pr-SS disrupt the binding  between Tem1 and Bub2 in vitro.	bind
15551	3	5473	7	10	NULL	NULL	NULL	Gic1-pr-SS	GP		disrupts					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_cellbiol_164_2_219_s_271	14734533	(G) Gic1-pr and Gic1-pr-SS disrupt the binding  between Tem1 and Bub2 in vitro.	bind
16373	1	5475	6	10	NULL	NULL	NULL	NSF	GP		does not bind					PICK1-SNAP complexes	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_34_1_53_s_127	11931741	(G) NSF does not bind PICK1-SNAP complexes.	bind
15552	1	5475	7	10	NULL	NULL	NULL	NSF	GP		does not bind					PICK1-SNAP complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_34_1_53_s_127	11931741	(G) NSF does not bind PICK1-SNAP complexes.	bind
16374	1	5476	6	10	NULL	NULL	NULL	PGL-1	GP		bind					laminin 2 chain	GP		LG1 module		NULL		NULL	NULL	NULL	NULL	gw60_cell_103_3_511_s_129	11081637	(G) PGL-1 binds  to LG1, LG4 and LG5 modules of the laminin  2 chain.	bind
16375	2	5476	6	10	NULL	NULL	NULL	PGL-1	GP		bind					laminin 2 chain	GP		LG4 module		NULL		NULL	NULL	NULL	NULL	gw60_cell_103_3_511_s_129	11081637	(G) PGL-1 binds  to LG1, LG4 and LG5 modules of the laminin  2 chain.	bind
16376	3	5476	6	10	NULL	NULL	NULL	PGL-1	GP		bind					laminin 2 chain	GP		LG5 module		NULL		NULL	NULL	NULL	NULL	gw60_cell_103_3_511_s_129	11081637	(G) PGL-1 binds  to LG1, LG4 and LG5 modules of the laminin  2 chain.	bind
15553	1	5476	7	10	NULL	NULL	NULL	PGL-1	GP		bind					laminin 2 chain	GP		LG1 module		NULL		NULL	NULL	NULL	NULL	gw60_cell_103_3_511_s_129	11081637	(G) PGL-1 binds  to LG1, LG4 and LG5 modules of the laminin  2 chain.	bind
15554	2	5476	7	10	NULL	NULL	NULL	PGL-1	GP		bind					laminin 2 chain	GP		LG4 module		NULL		NULL	NULL	NULL	NULL	gw60_cell_103_3_511_s_129	11081637	(G) PGL-1 binds  to LG1, LG4 and LG5 modules of the laminin  2 chain.	bind
15555	3	5476	7	10	NULL	NULL	NULL	PGL-1	GP		bind					laminin 2 chain	GP		LG5 module		NULL		NULL	NULL	NULL	NULL	gw60_cell_103_3_511_s_129	11081637	(G) PGL-1 binds  to LG1, LG4 and LG5 modules of the laminin  2 chain.	bind
16377	1	5477	6	10	NULL	NULL	NULL	Skp1p	GP		bind					sgt1-5 protein	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_molcell_4_1_21_s_145	10445024	(G) Skp1p binds to  sgt1-5 mutant protein, but not  sgt1-3 mutant protein.	bind
16378	2	5477	6	10	NULL	NULL	NULL	Skp1p	GP		does not bind					sgt1-3 protein	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_molcell_4_1_21_s_145	10445024	(G) Skp1p binds to  sgt1-5 mutant protein, but not  sgt1-3 mutant protein.	bind
15556	1	5477	7	10	NULL	NULL	NULL	 Skp1p	GP		bind					 sgt1-5	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_molcell_4_1_21_s_145	10445024	(G) Skp1p binds to  sgt1-5 mutant protein, but not  sgt1-3 mutant protein.	bind
15557	2	5477	7	10	NULL	NULL	NULL	Skp1p	GP		does not bind					sgt1-3	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_molcell_4_1_21_s_145	10445024	(G) Skp1p binds to  sgt1-5 mutant protein, but not  sgt1-3 mutant protein.	bind
16379	1	5479	6	10	NULL	NULL	NULL	KSRP	GP		bind		specifically			RNA	NucleicAcid			AREfos	NULL		NULL	NULL	NULL	NULL	gw60_cell_107_4_451_s_229	11719186	(G) Specific binding of KSRP to  AREfos RNA.	bind
15558	1	5479	7	10	NULL	NULL	NULL	KSRP	GP		bind		specifically			  RNA	NucleicAcid			AREfos	NULL		NULL	NULL	NULL	NULL	gw60_cell_107_4_451_s_229	11719186	(G) Specific binding of KSRP to  AREfos RNA.	bind
16384	1	5481	6	10	NULL	NULL	NULL	Raichu-RhoA	GP		bind					GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_166_7_975_s_98	15452141	(G), Schematic representations of Raichu-RhoA bound to GDP  or GTP.	bind
16385	2	5481	6	10	NULL	NULL	NULL	Raichu-RhoA	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_166_7_975_s_98	15452141	(G), Schematic representations of Raichu-RhoA bound to GDP  or GTP.	bind
16386	3	5481	6	10	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_166_7_975_s_98	15452141	(G), Schematic representations of Raichu-RhoA bound to GDP  or GTP.	bind
15559	1	5481	7	10	NULL	NULL	NULL	Raichu-RhoA	GP		bind					GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_166_7_975_s_98	15452141	(G), Schematic representations of Raichu-RhoA bound to GDP  or GTP.	bind
15560	2	5481	7	10	NULL	NULL	NULL	Raichu-RhoA	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_166_7_975_s_98	15452141	(G), Schematic representations of Raichu-RhoA bound to GDP  or GTP.	bind
19614	3	5481	7	10	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_166_7_975_s_98	15452141	(G), Schematic representations of Raichu-RhoA bound to GDP  or GTP.	bind
16387	1	5486	6	10	NULL	NULL	NULL	HSF1	GP		bind									HSE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_4949_s_223	9710578	(GA) enhances the heat-inducible HSE-binding activity of HSF1 and delays deactivation during recovery.	bind
16388	2	5486	6	10	NULL	NULL	NULL	statement 1	Process		is induced by					Heat					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_4949_s_223	9710578	(GA) enhances the heat-inducible HSE-binding activity of HSF1 and delays deactivation during recovery.	bind
16389	3	5486	6	10	NULL	NULL	NULL	GA	Chemical		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_4949_s_223	9710578	(GA) enhances the heat-inducible HSE-binding activity of HSF1 and delays deactivation during recovery.	bind
19615	1	5486	7	10	NULL	NULL	NULL				bind				HSE	HSF1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_4949_s_223	9710578	(GA) enhances the heat-inducible HSE-binding activity of HSF1 and delays deactivation during recovery.	bind
19616	2	5486	7	10	NULL	NULL	NULL	statement 1	Process		is induced by					heat					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_4949_s_223	9710578	(GA) enhances the heat-inducible HSE-binding activity of HSF1 and delays deactivation during recovery.	bind
19617	3	5486	7	10	NULL	NULL	NULL	GA	Chemical		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_4949_s_223	9710578	(GA) enhances the heat-inducible HSE-binding activity of HSF1 and delays deactivation during recovery.	bind
16390	1	5487	6	10	NULL	NULL	NULL	GAL4	GP		bind									CGGN11CCG	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5279_s_124	10409719	(GAL4 binds to the sequence CGGN11CCG, and PUT3 binds the sequence CGGN10CCG [ 49].)	bind
16391	2	5487	6	10	NULL	NULL	NULL	PUT3	GP		bind									CGGN10CCG	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5279_s_124	10409719	(GAL4 binds to the sequence CGGN11CCG, and PUT3 binds the sequence CGGN10CCG [ 49].)	bind
15563	1	5487	7	10	NULL	NULL	NULL	GAL4	GP		bind									CGGN11CCG	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5279_s_124	10409719	(GAL4 binds to the sequence CGGN11CCG, and PUT3 binds the sequence CGGN10CCG [ 49].)	bind
15564	2	5487	7	10	NULL	NULL	NULL	PUT3	GP		bind									CGGN10CCG	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5279_s_124	10409719	(GAL4 binds to the sequence CGGN11CCG, and PUT3 binds the sequence CGGN10CCG [ 49].)	bind
16392	1	5488	6	10	NULL	NULL	NULL	GAL4-VP16	GP		bind					linker DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_14773_s_162	11279013	(GAL4-VP16 binding to linker DNA protects it from MNase digestion and increases the yield of fragments corresponding to dinucleosomes).	bind
16393	2	5488	6	10	NULL	NULL	NULL	MNase	GP		digests					linker DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_14773_s_162	11279013	(GAL4-VP16 binding to linker DNA protects it from MNase digestion and increases the yield of fragments corresponding to dinucleosomes).	bind
16394	3	5488	6	10	NULL	NULL	NULL	statement 1	Process		protects					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_14773_s_162	11279013	(GAL4-VP16 binding to linker DNA protects it from MNase digestion and increases the yield of fragments corresponding to dinucleosomes).	bind
16395	4	5488	6	10	NULL	NULL	NULL	GAL4-VP16	GP		increases					dinucleosome fragments	CellComponent	yield of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_14773_s_162	11279013	(GAL4-VP16 binding to linker DNA protects it from MNase digestion and increases the yield of fragments corresponding to dinucleosomes).	bind
15565	1	5488	7	10	NULL	NULL	NULL	GAL4-VP16	GP		bind					linker DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_14773_s_162	11279013	(GAL4-VP16 binding to linker DNA protects it from MNase digestion and increases the yield of fragments corresponding to dinucleosomes).	bind
15566	4	5488	7	10	NULL	NULL	NULL	statement 1	Process		protects					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_14773_s_162	11279013	(GAL4-VP16 binding to linker DNA protects it from MNase digestion and increases the yield of fragments corresponding to dinucleosomes).	bind
15567	3	5488	7	10	NULL	NULL	NULL	statement 1	Process		increases					dinucleosome fragments	CellComponent	yield of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_14773_s_162	11279013	(GAL4-VP16 binding to linker DNA protects it from MNase digestion and increases the yield of fragments corresponding to dinucleosomes).	bind
44828	2	5488	7	10	NULL	NULL	NULL	linker DNA	NucleicAcid		digest					MNase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_14773_s_162	11279013	(GAL4-VP16 binding to linker DNA protects it from MNase digestion and increases the yield of fragments corresponding to dinucleosomes).	bind
16396	1	5490	6	10	NULL	NULL	NULL	Oct4	GP		bind									composite sox-oct element	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_14_6031_s_276	15988017	(H) Analysis of the cooperativity of Oct4 and Sox2 binding  to the composite sox-oct element.	bind
16397	2	5490	6	10	NULL	NULL	NULL	Sox2	GP		bind									composite sox-oct element	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_14_6031_s_276	15988017	(H) Analysis of the cooperativity of Oct4 and Sox2 binding  to the composite sox-oct element.	bind
16398	3	5490	6	10	NULL	NULL	NULL	statement 1	Process		acts in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_14_6031_s_276	15988017	(H) Analysis of the cooperativity of Oct4 and Sox2 binding  to the composite sox-oct element.	bind
15568	1	5490	7	10	NULL	NULL	NULL	Oct4	GP		bind									composite sox-oct  element	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_14_6031_s_276	15988017	(H) Analysis of the cooperativity of Oct4 and Sox2 binding  to the composite sox-oct element.	bind
15569	2	5490	7	10	NULL	NULL	NULL	Sox2	GP		bind									composite sox-oct element	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_14_6031_s_276	15988017	(H) Analysis of the cooperativity of Oct4 and Sox2 binding  to the composite sox-oct element.	bind
15570	3	5490	7	10	NULL	NULL	NULL	statement 1	Process		occurs in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_14_6031_s_276	15988017	(H) Analysis of the cooperativity of Oct4 and Sox2 binding  to the composite sox-oct element.	bind
16399	1	5491	6	10	NULL	NULL	NULL	anti-CD34	GP	mouse	bind					tumor cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_science_279_5350_577_s_47	9438854	(H) Binding of mouse anti-CD34 to tumor cells demonstrated by RPE-labeled anti-mouse IgG (red).	bind
15571	1	5491	7	10	NULL	NULL	NULL	anti-CD34	GP	mouse	bind					tumor cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_science_279_5350_577_s_47	9438854	(H) Binding of mouse anti-CD34 to tumor cells demonstrated by RPE-labeled anti-mouse IgG (red).	bind
16400	1	5492	6	10	NULL	NULL	NULL	Dlt	GP		bind		directly			Par-6	GP				NULL		NULL	NULL	NULL	NULL	gw60_development_130_18_4363_s_166	12900452	(H) Direct binding of Dlt to Par-6, but not to aPKC or Baz.	bind
16401	2	5492	6	10	NULL	NULL	NULL	Dlt	GP		does not bind					aPKC	GP				NULL		NULL	NULL	NULL	NULL	gw60_development_130_18_4363_s_166	12900452	(H) Direct binding of Dlt to Par-6, but not to aPKC or Baz.	bind
16402	3	5492	6	10	NULL	NULL	NULL	Dlt	GP		does not bind					Baz	GP				NULL		NULL	NULL	NULL	NULL	gw60_development_130_18_4363_s_166	12900452	(H) Direct binding of Dlt to Par-6, but not to aPKC or Baz.	bind
15572	1	5492	7	10	NULL	NULL	NULL	Dlt 	GP		bind		directly			Par-6	GP				NULL		NULL	NULL	NULL	NULL	gw60_development_130_18_4363_s_166	12900452	(H) Direct binding of Dlt to Par-6, but not to aPKC or Baz.	bind
15573	2	5492	7	10	NULL	NULL	NULL	Dlt	GP		does not bind					PKC	GP				NULL		NULL	NULL	NULL	NULL	gw60_development_130_18_4363_s_166	12900452	(H) Direct binding of Dlt to Par-6, but not to aPKC or Baz.	bind
15574	3	5492	7	10	NULL	NULL	NULL	Dlt	GP		does not bind					Baz	GP				NULL		NULL	NULL	NULL	NULL	gw60_development_130_18_4363_s_166	12900452	(H) Direct binding of Dlt to Par-6, but not to aPKC or Baz.	bind
16403	1	5493	6	10	NULL	NULL	NULL	Pit1	GP		bind					TSHbeta 	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_cell_97_5_587_s_145	10367888	(H) DNA binding of Pit1  and GATA2 on the  TSHbeta promoter.	bind
16404	2	5493	6	10	NULL	NULL	NULL	GATA2	GP		bind					TSHbeta	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_cell_97_5_587_s_145	10367888	(H) DNA binding of Pit1  and GATA2 on the  TSHbeta promoter.	bind
15575	1	5493	7	10	NULL	NULL	NULL	Pit1 	GP		bind					 TSHbeta	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_cell_97_5_587_s_145	10367888	(H) DNA binding of Pit1  and GATA2 on the  TSHbeta promoter.	bind
15576	2	5493	7	10	NULL	NULL	NULL	GATA2	GP		bind					TSHbeta	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_cell_97_5_587_s_145	10367888	(H) DNA binding of Pit1  and GATA2 on the  TSHbeta promoter.	bind
16405	1	5495	6	10	NULL	NULL	NULL	Wg	GP		expressed in					Wing	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_development_130_17_4135_s_372	12874133	(H) Expression of UAS- dve with  sd-Gal4 abolishes expression of Wg in the wing.	bind
16406	2	5495	6	10	NULL	NULL	NULL	UAS-dve	GP	expression of	occurs simultaneously with					Sd-Gal4	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_development_130_17_4135_s_372	12874133	(H) Expression of UAS- dve with  sd-Gal4 abolishes expression of Wg in the wing.	bind
16407	3	5495	6	10	NULL	NULL	NULL	statement 2	Process		abolishes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_development_130_17_4135_s_372	12874133	(H) Expression of UAS- dve with  sd-Gal4 abolishes expression of Wg in the wing.	bind
15577	2	5495	7	10	NULL	NULL	NULL	Wg	GP		is expressed in					wing	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_development_130_17_4135_s_372	12874133	(H) Expression of UAS- dve with  sd-Gal4 abolishes expression of Wg in the wing.	bind
15578	1	5495	7	10	NULL	NULL	NULL	UAS- dve	GP	expression of	occurs simultaneously with					sd-Gal4	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_development_130_17_4135_s_372	12874133	(H) Expression of UAS- dve with  sd-Gal4 abolishes expression of Wg in the wing.	bind
53104	3	5495	7	10	NULL	NULL	NULL	statement 1	Process		abolishes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_development_130_17_4135_s_372	12874133	(H) Expression of UAS- dve with  sd-Gal4 abolishes expression of Wg in the wing.	bind
16408	1	5496	6	10	NULL	NULL	NULL	Hp1	GP		bind					lineage progenitors	Cell	MAA-positive			NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_3_263_s_119	10198629	(H) Hp1 (yellow) binding to MAA-positive lineage progenitors (green) that predominate in normal, embryonic day 18.5 FVB/N gastric epithelium.	bind
16409	2	5496	6	10	NULL	NULL	NULL	lineage progenitors	Cell	MAA-positive	predominate in					embryonic day 18.5 FVB/N gastric epithelium	OrganismPart	normal			NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_3_263_s_119	10198629	(H) Hp1 (yellow) binding to MAA-positive lineage progenitors (green) that predominate in normal, embryonic day 18.5 FVB/N gastric epithelium.	bind
15579	1	5496	7	10	NULL	NULL	NULL	Hp1	GP		bind					lineage progenitors	Cell	MAA-positive			NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_3_263_s_119	10198629	(H) Hp1 (yellow) binding to MAA-positive lineage progenitors (green) that predominate in normal, embryonic day 18.5 FVB/N gastric epithelium.	bind
19618	2	5496	7	10	NULL	NULL	NULL	lineage progenitors	Cell	MAA-positive	predominate in					embryonic day 18.5 FVB/N gastric epithelium	OrganismPart	normal			NULL		NULL	NULL	NULL	NULL	gw60_molcell_3_3_263_s_119	10198629	(H) Hp1 (yellow) binding to MAA-positive lineage progenitors (green) that predominate in normal, embryonic day 18.5 FVB/N gastric epithelium.	bind
16410	1	5497	6	10	NULL	NULL	NULL	centrin 2	GP	human	bind					hSfi1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_162_7_1211_s_166	14504268	(h) Human centrin 2 binding  to GST fusions of hSfi1.	bind
44792	2	5497	6	10	NULL	NULL	NULL	hSfi1	GP		is a type of					GST fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_162_7_1211_s_166	14504268	(h) Human centrin 2 binding  to GST fusions of hSfi1.	bind
15580	1	5497	7	10	NULL	NULL	NULL	centrin 2 	GP	human	bind					hSfi1	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_162_7_1211_s_166	14504268	(h) Human centrin 2 binding  to GST fusions of hSfi1.	bind
44793	2	5497	7	10	NULL	NULL	NULL	hSfi1	GP		is a type of					GST fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_162_7_1211_s_166	14504268	(h) Human centrin 2 binding  to GST fusions of hSfi1.	bind
16448	1	5498	6	10	NULL	NULL	NULL	p53	GP		bind		directly			myosin VI	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_6_2175_s_151	16507995	(H) p53 binds directly to the myosin  VI promoter.	bind
15581	1	5498	7	10	NULL	NULL	NULL	p53	GP		binds		directly			myosin VI	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_6_2175_s_151	16507995	(H) p53 binds directly to the myosin  VI promoter.	bind
16510	1	5499	6	10	NULL	NULL	NULL	Pros-S	GP		bind									seq56B	NULL		NULL	NULL	NULL	NULL	gw60_devcell_4_6_853_s_111	12791270	(H) Pros-S binding to seq56B.	bind
15582	1	5499	7	10	NULL	NULL	NULL	Pros-S	GP		bind									seq56B	NULL		NULL	NULL	NULL	NULL	gw60_devcell_4_6_853_s_111	12791270	(H) Pros-S binding to seq56B.	bind
16511	1	5500	6	10	NULL	NULL	NULL	Patr-B0101	GP		bind								I1452V variant		NULL		NULL	NULL	NULL	NULL	gw60_immunity_15_6_883_s_135	11754811	(H) Relative binding capacity to Patr-B0101 binding of the I1452V or D1449E variants and the NS31444 parental peptide.	bind
16512	2	5500	6	10	NULL	NULL	NULL	Patr-B0101	GP		bind								D1449E variant		NULL		NULL	NULL	NULL	NULL	gw60_immunity_15_6_883_s_135	11754811	(H) Relative binding capacity to Patr-B0101 binding of the I1452V or D1449E variants and the NS31444 parental peptide.	bind
16513	3	5500	6	10	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_15_6_883_s_135	11754811	(H) Relative binding capacity to Patr-B0101 binding of the I1452V or D1449E variants and the NS31444 parental peptide.	bind
16514	4	5500	6	10	NULL	NULL	NULL	Patr-B0101	GP		bind					NS31444 parental peptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_15_6_883_s_135	11754811	(H) Relative binding capacity to Patr-B0101 binding of the I1452V or D1449E variants and the NS31444 parental peptide.	bind
15782	1	5500	7	10	NULL	NULL	NULL				bind			I1452V		 Patr-B0101	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_15_6_883_s_135	11754811	(H) Relative binding capacity to Patr-B0101 binding of the I1452V or D1449E variants and the NS31444 parental peptide.	bind
15783	2	5500	7	10	NULL	NULL	NULL				bind			D1449E 		Patr-B0101	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_15_6_883_s_135	11754811	(H) Relative binding capacity to Patr-B0101 binding of the I1452V or D1449E variants and the NS31444 parental peptide.	bind
15784	3	5500	7	10	NULL	NULL	NULL	NS31444 parental peptide	GP		bind					Patr-B0101	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_15_6_883_s_135	11754811	(H) Relative binding capacity to Patr-B0101 binding of the I1452V or D1449E variants and the NS31444 parental peptide.	bind
44794	4	5500	7	10	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_15_6_883_s_135	11754811	(H) Relative binding capacity to Patr-B0101 binding of the I1452V or D1449E variants and the NS31444 parental peptide.	bind
16515	1	5501	6	10	NULL	NULL	NULL	Yan	GP		bind									ETS domain binding sites 1 within SME	NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_161	11051549	(H) Yan binds to ETS domain binding  sites 1, 2, 4, and 6 within the SME, causing shifted bands.	bind
16516	2	5501	6	10	NULL	NULL	NULL	Yan	GP		bind									ETS domain binding sites 2 within SME	NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_161	11051549	(H) Yan binds to ETS domain binding  sites 1, 2, 4, and 6 within the SME, causing shifted bands.	bind
16517	3	5501	6	10	NULL	NULL	NULL	Yan	GP		bind									ETS domain binding sites 4 within SME	NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_161	11051549	(H) Yan binds to ETS domain binding  sites 1, 2, 4, and 6 within the SME, causing shifted bands.	bind
16518	4	5501	6	10	NULL	NULL	NULL	Yan	GP		bind									ETS domain binding sites 6 within SME	NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_161	11051549	(H) Yan binds to ETS domain binding  sites 1, 2, 4, and 6 within the SME, causing shifted bands.	bind
15778	1	5501	7	10	NULL	NULL	NULL	Yan	GP		bind									ETS domain 1 within SME	NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_161	11051549	(H) Yan binds to ETS domain binding  sites 1, 2, 4, and 6 within the SME, causing shifted bands.	bind
15779	2	5501	7	10	NULL	NULL	NULL	Yan 	GP		bind									ETS domain 2 within SME	NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_161	11051549	(H) Yan binds to ETS domain binding  sites 1, 2, 4, and 6 within the SME, causing shifted bands.	bind
15780	3	5501	7	10	NULL	NULL	NULL	Yan	GP		bind									ETS domain 4 within SME	NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_161	11051549	(H) Yan binds to ETS domain binding  sites 1, 2, 4, and 6 within the SME, causing shifted bands.	bind
15781	4	5501	7	10	NULL	NULL	NULL	Yan	GP		bind									ETS domain 6 within SME	NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_161	11051549	(H) Yan binds to ETS domain binding  sites 1, 2, 4, and 6 within the SME, causing shifted bands.	bind
16519	1	5502	6	10	NULL	NULL	NULL	dTCF-HMG protein	GP		bind					wing	OrganismPart			794 bp Ser of enhancer	NULL		NULL	NULL	NULL	NULL	gw70_development_131_2_285_s_165	14701680	(H-K) DNase I footprinting analysis of the  dTCF-HMG protein bound to the 794 bp  Ser wing enhancer.	bind
15785	1	5502	7	10	NULL	NULL	NULL	dTCF-HMG protein	GP		bind					wing	OrganismPart			794 bp Ser of enhancer	NULL		NULL	NULL	NULL	NULL	gw70_development_131_2_285_s_165	14701680	(H-K) DNase I footprinting analysis of the  dTCF-HMG protein bound to the 794 bp  Ser wing enhancer.	bind
16520	1	5506	6	10	NULL	NULL	NULL				bind			K3L		PKR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_2_295_s_234	12191475	(His 47), also reduced the binding affinity of K3L for PKR.	bind
67197	2	5506	6	10	NULL	NULL	NULL				reduce			His 47		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_2_295_s_234	12191475	(His 47), also reduced the binding affinity of K3L for PKR.	bind
15786	1	5506	7	10	NULL	NULL	NULL				bind			K3L		PKR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_2_295_s_234	12191475	(His 47), also reduced the binding affinity of K3L for PKR.	bind
15787	2	5506	7	10	NULL	NULL	NULL				reduce			His 47		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_2_295_s_234	12191475	(His 47), also reduced the binding affinity of K3L for PKR.	bind
16521	1	5508	6	10	NULL	NULL	NULL				does not bind			His- lC		F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_33_23549_s_205	10438535	(His- lC) does not bind to F-actin in the co-sedimentation assay excludes the tag as a mediator of F-actin binding.	bind
15788	1	5508	7	10	NULL	NULL	NULL				does not bind			His- lC		F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_33_23549_s_205	10438535	(His- lC) does not bind to F-actin in the co-sedimentation assay excludes the tag as a mediator of F-actin binding.	bind
16522	1	5509	6	10	NULL	NULL	NULL	HSF	GP		bind									heat shock element	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_7_792_s_131	10766736	(HSE) The heat shock element to which HSF binds; (GA) a GAGA element to which GAGA factor binds (Wilkins and Lis 1997  ).	bind
16523	2	5509	6	10	NULL	NULL	NULL	GAGA factor	GP		bind									GAGA element	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_7_792_s_131	10766736	(HSE) The heat shock element to which HSF binds; (GA) a GAGA element to which GAGA factor binds (Wilkins and Lis 1997  ).	bind
15789	1	5509	7	10	NULL	NULL	NULL	HSF	GP		bind									heat shock element	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_7_792_s_131	10766736	(HSE) The heat shock element to which HSF binds; (GA) a GAGA element to which GAGA factor binds (Wilkins and Lis 1997  ).	bind
15790	2	5509	7	10	NULL	NULL	NULL	GAGA factor	GP		bind									GAGA element	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_7_792_s_131	10766736	(HSE) The heat shock element to which HSF binds; (GA) a GAGA element to which GAGA factor binds (Wilkins and Lis 1997  ).	bind
16524	1	5511	6	10	NULL	NULL	NULL	GST-EB1	GP		bind					Mlp-FLAG	GP				NULL	SF9 whole cell extracts	NULL	NULL	NULL	NULL	gw70_cellbiol_171_2_201_s_104	16247022	(I and J) GST-EB1 but not GST binds Mlp-FLAG whether present in SF9 whole  cell extracts	bind
16525	2	5511	6	10	NULL	NULL	NULL	GST	Chemical		does not bind					Mlp-FLAG	GP				NULL	SF9 whole cell extracts	NULL	NULL	NULL	NULL	gw70_cellbiol_171_2_201_s_104	16247022	(I and J) GST-EB1 but not GST binds Mlp-FLAG whether present in SF9 whole  cell extracts	bind
15791	1	5511	7	10	NULL	NULL	NULL	GST-EB1	GP		bind					Mlp-FLAG	GP				NULL	 SF9 whole cell extracts	NULL	NULL	NULL	NULL	gw70_cellbiol_171_2_201_s_104	16247022	(I and J) GST-EB1 but not GST binds Mlp-FLAG whether present in SF9 whole  cell extracts	bind
15792	2	5511	7	10	NULL	NULL	NULL	GST	Chemical		does not bind					Mlp-FLAG	GP				NULL	SF9 whole cell extracts	NULL	NULL	NULL	NULL	gw70_cellbiol_171_2_201_s_104	16247022	(I and J) GST-EB1 but not GST binds Mlp-FLAG whether present in SF9 whole  cell extracts	bind
16526	1	5512	6	10	NULL	NULL	NULL	P450 2E1	GP		bind					ethanol	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_34_23833_s_173	10446146	(i)  K d values for binding of P450 2E1 and either ethanol, acetaldehyde, or acetic acid are all high (millimolar to molar range).	bind
16527	2	5512	6	10	NULL	NULL	NULL	P450 2E1	GP		bind					acetaldehyde	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_34_23833_s_173	10446146	(i)  K d values for binding of P450 2E1 and either ethanol, acetaldehyde, or acetic acid are all high (millimolar to molar range).	bind
16528	3	5512	6	10	NULL	NULL	NULL	P450 2E1	GP		bind					acetic acid	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_34_23833_s_173	10446146	(i)  K d values for binding of P450 2E1 and either ethanol, acetaldehyde, or acetic acid are all high (millimolar to molar range).	bind
16301	1	5512	7	10	NULL	NULL	NULL	P450 2E1	GP		bind					ethanol	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_34_23833_s_173	10446146	(i)  K d values for binding of P450 2E1 and either ethanol, acetaldehyde, or acetic acid are all high (millimolar to molar range).	bind
16302	2	5512	7	10	NULL	NULL	NULL	P450 2E1	GP		bind					acetaldehyde	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_34_23833_s_173	10446146	(i)  K d values for binding of P450 2E1 and either ethanol, acetaldehyde, or acetic acid are all high (millimolar to molar range).	bind
16303	3	5512	7	10	NULL	NULL	NULL	P450 2E1	GP		bind					acetic acid	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_34_23833_s_173	10446146	(i)  K d values for binding of P450 2E1 and either ethanol, acetaldehyde, or acetic acid are all high (millimolar to molar range).	bind
16529	1	5513	6	10	NULL	NULL	NULL	MAQ1	GP		bind					P-TEFb	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_14_4859_s_370	12832472	(i) 7SK RNA is essential for MAQ1 binding to P-TEFb, whereas although TAR RNA enhances the interaction between Tat and cyclin T1 ( 63), Tat binding to P-TEFb can occur in the absence of TAR RNA ( 25,  61).	bind
16530	2	5513	6	10	NULL	NULL	NULL	7SK RNA	NucleicAcid		is essential for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_14_4859_s_370	12832472	(i) 7SK RNA is essential for MAQ1 binding to P-TEFb, whereas although TAR RNA enhances the interaction between Tat and cyclin T1 ( 63), Tat binding to P-TEFb can occur in the absence of TAR RNA ( 25,  61).	bind
16531	3	5513	6	10	NULL	NULL	NULL	Tat	GP		bind					cyclin T1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_14_4859_s_370	12832472	(i) 7SK RNA is essential for MAQ1 binding to P-TEFb, whereas although TAR RNA enhances the interaction between Tat and cyclin T1 ( 63), Tat binding to P-TEFb can occur in the absence of TAR RNA ( 25,  61).	bind
16532	4	5513	6	10	NULL	NULL	NULL	Tat	GP		bind					P-TEFb	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_14_4859_s_370	12832472	(i) 7SK RNA is essential for MAQ1 binding to P-TEFb, whereas although TAR RNA enhances the interaction between Tat and cyclin T1 ( 63), Tat binding to P-TEFb can occur in the absence of TAR RNA ( 25,  61).	bind
16533	5	5513	6	10	NULL	NULL	NULL	statement 4	Process		occur in the absence of					TAR RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_14_4859_s_370	12832472	(i) 7SK RNA is essential for MAQ1 binding to P-TEFb, whereas although TAR RNA enhances the interaction between Tat and cyclin T1 ( 63), Tat binding to P-TEFb can occur in the absence of TAR RNA ( 25,  61).	bind
16534	6	5513	6	10	NULL	NULL	NULL	TAR RNA	NucleicAcid		enhances					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_14_4859_s_370	12832472	(i) 7SK RNA is essential for MAQ1 binding to P-TEFb, whereas although TAR RNA enhances the interaction between Tat and cyclin T1 ( 63), Tat binding to P-TEFb can occur in the absence of TAR RNA ( 25,  61).	bind
15793	1	5513	7	10	NULL	NULL	NULL	MAQ1 	GP		bind					P-TEFb	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_14_4859_s_370	12832472	(i) 7SK RNA is essential for MAQ1 binding to P-TEFb, whereas although TAR RNA enhances the interaction between Tat and cyclin T1 ( 63), Tat binding to P-TEFb can occur in the absence of TAR RNA ( 25,  61).	bind
15794	2	5513	7	10	NULL	NULL	NULL	7SK RNA	NucleicAcid		is essential for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_14_4859_s_370	12832472	(i) 7SK RNA is essential for MAQ1 binding to P-TEFb, whereas although TAR RNA enhances the interaction between Tat and cyclin T1 ( 63), Tat binding to P-TEFb can occur in the absence of TAR RNA ( 25,  61).	bind
15795	3	5513	7	10	NULL	NULL	NULL	 Tat	GP		bind					cyclin T1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_14_4859_s_370	12832472	(i) 7SK RNA is essential for MAQ1 binding to P-TEFb, whereas although TAR RNA enhances the interaction between Tat and cyclin T1 ( 63), Tat binding to P-TEFb can occur in the absence of TAR RNA ( 25,  61).	bind
15796	4	5513	7	10	NULL	NULL	NULL	 TAR RNA	NucleicAcid		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_14_4859_s_370	12832472	(i) 7SK RNA is essential for MAQ1 binding to P-TEFb, whereas although TAR RNA enhances the interaction between Tat and cyclin T1 ( 63), Tat binding to P-TEFb can occur in the absence of TAR RNA ( 25,  61).	bind
15797	5	5513	7	10	NULL	NULL	NULL	Tat	GP		bind					P-TEFb	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_14_4859_s_370	12832472	(i) 7SK RNA is essential for MAQ1 binding to P-TEFb, whereas although TAR RNA enhances the interaction between Tat and cyclin T1 ( 63), Tat binding to P-TEFb can occur in the absence of TAR RNA ( 25,  61).	bind
15798	6	5513	7	10	NULL	NULL	NULL	statement 5	Process		occur in the absence of					TAR RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_14_4859_s_370	12832472	(i) 7SK RNA is essential for MAQ1 binding to P-TEFb, whereas although TAR RNA enhances the interaction between Tat and cyclin T1 ( 63), Tat binding to P-TEFb can occur in the absence of TAR RNA ( 25,  61).	bind
16535	1	5515	6	10	NULL	NULL	NULL	GST-L18	GP		bind		directly			PKR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_2_1116_s_290	9891046	(i) A GST-L18 fusion protein directly bound to PKR.	bind
44806	2	5515	6	10	NULL	NULL	NULL	GST-L18 	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_2_1116_s_290	9891046	(i) A GST-L18 fusion protein directly bound to PKR.	bind
15799	1	5515	7	10	NULL	NULL	NULL	GST-L18	GP		bind		directly			PKR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_2_1116_s_290	9891046	(i) A GST-L18 fusion protein directly bound to PKR.	bind
44807	2	5515	7	10	NULL	NULL	NULL	GST-L18 	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_2_1116_s_290	9891046	(i) A GST-L18 fusion protein directly bound to PKR.	bind
16536	1	5516	6	10	NULL	NULL	NULL	antibodies	GP		bind					Vn	GP	close proximity to	cell adhesion domain		NULL	unfractionated plasma	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_21_13705_s_6	9153222	(i) Antibodies that bind in close proximity to the cell adhesion domain of Vn fail to bind to native Vn present in unfractionated plasma.	bind
16537	2	5516	6	10	NULL	NULL	NULL	antibodies	GP		does not bind					Vn	GP	native			NULL	unfractionated plasma	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_21_13705_s_6	9153222	(i) Antibodies that bind in close proximity to the cell adhesion domain of Vn fail to bind to native Vn present in unfractionated plasma.	bind
15800	1	5516	7	10	NULL	NULL	NULL	Antibodies	GP		bind					Vn 	GP	close proximity to	cell adhesion domain		NULL	unfractionated plasma	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_21_13705_s_6	9153222	(i) Antibodies that bind in close proximity to the cell adhesion domain of Vn fail to bind to native Vn present in unfractionated plasma.	bind
15802	3	5516	7	10	NULL	NULL	NULL	Antibodies	GP		does not bind					Vn	GP	native			NULL	 unfractionated plasma	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_21_13705_s_6	9153222	(i) Antibodies that bind in close proximity to the cell adhesion domain of Vn fail to bind to native Vn present in unfractionated plasma.	bind
16538	1	5517	6	10	NULL	NULL	NULL	AP-Sema3A	GP		bind		high affinity			corpus callosum axons	OrganismPart				NULL	E17.5 wild type mice	NULL	NULL	NULL	NULL	gw60_devcell_5_1_45_s_156	12852851	(I) AP-Sema3A section binding reveals a high level of Sema3A binding to axons of the E17.5 corpus callosum in wild-type mice.	bind
15803	1	5517	7	10	NULL	NULL	NULL	AP-Sema3A	GP		bind		high affinity			corpus callosum axons	OrganismPart				NULL	E17.5  wild-type mice	NULL	NULL	NULL	NULL	gw60_devcell_5_1_45_s_156	12852851	(I) AP-Sema3A section binding reveals a high level of Sema3A binding to axons of the E17.5 corpus callosum in wild-type mice.	bind
16539	1	5518	6	10	NULL	NULL	NULL	ATP	Chemical		bind								D1 domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_90_3_523_s_122	9267032	(i) ATP  bound to both D1 and D2 domains maintains the closed cylinder.	bind
16540	2	5518	6	10	NULL	NULL	NULL	ATP	Chemical		bind								D2 domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_90_3_523_s_122	9267032	(i) ATP  bound to both D1 and D2 domains maintains the closed cylinder.	bind
16541	3	5518	6	10	NULL	NULL	NULL	statement 1	Process		occurs simultaneously with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_90_3_523_s_122	9267032	(i) ATP  bound to both D1 and D2 domains maintains the closed cylinder.	bind
16542	4	5518	6	10	NULL	NULL	NULL	statement 3	Process		maintains					closed cylinder					NULL		NULL	NULL	NULL	NULL	gw60_cell_90_3_523_s_122	9267032	(i) ATP  bound to both D1 and D2 domains maintains the closed cylinder.	bind
15804	1	5518	7	10	NULL	NULL	NULL	ATP	Chemical		bind								D1 domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_90_3_523_s_122	9267032	(i) ATP  bound to both D1 and D2 domains maintains the closed cylinder.	bind
15805	2	5518	7	10	NULL	NULL	NULL	ATP	Chemical		bind								D2 domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_90_3_523_s_122	9267032	(i) ATP  bound to both D1 and D2 domains maintains the closed cylinder.	bind
15806	3	5518	7	10	NULL	NULL	NULL	statement 1	Process		occurs simultaneously with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_90_3_523_s_122	9267032	(i) ATP  bound to both D1 and D2 domains maintains the closed cylinder.	bind
15807	4	5518	7	10	NULL	NULL	NULL	statement 3	Process		maintains					closed cylinder					NULL		NULL	NULL	NULL	NULL	gw60_cell_90_3_523_s_122	9267032	(i) ATP  bound to both D1 and D2 domains maintains the closed cylinder.	bind
16543	1	5519	6	10	NULL	NULL	NULL	PrPSc	GP		bind					PrP-Fc2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_113_1_49_s_160	12679034	(I) Binding of PrPSc to PrP-Fc2 is highly sensitive to chaotropic salts.	bind
16544	2	5519	6	10	NULL	NULL	NULL	statement 1	Process		is sensitive to 		highly			chaotropic salts	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_113_1_49_s_160	12679034	(I) Binding of PrPSc to PrP-Fc2 is highly sensitive to chaotropic salts.	bind
15808	1	5519	7	10	NULL	NULL	NULL	PrPSc	GP		bind					PrP-Fc2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_113_1_49_s_160	12679034	(I) Binding of PrPSc to PrP-Fc2 is highly sensitive to chaotropic salts.	bind
15809	2	5519	7	10	NULL	NULL	NULL	statement 1	Process		is sensitive to		highly			chaotropic salts	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_113_1_49_s_160	12679034	(I) Binding of PrPSc to PrP-Fc2 is highly sensitive to chaotropic salts.	bind
16545	1	5520	6	10	NULL	NULL	NULL	Cu(I)	Chemical		bind					chaperone	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_25_23163_s_256	12686548	(i) Can the two-coordinate Cu(I)-bound chaperone ever be  prepared free from ligation by an exogenous third ligand, and if so, what is  the structure?	bind
15810	1	5520	7	10	NULL	NULL	NULL	chaperone	GP		bind					Cu(I)	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_25_23163_s_256	12686548	(i) Can the two-coordinate Cu(I)-bound chaperone ever be  prepared free from ligation by an exogenous third ligand, and if so, what is  the structure?	bind
16546	1	5521	6	10	NULL	NULL	NULL	glucose catabolites	Chemical		activate					HPr kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_64_7_2513_s_193	9647823	(i) Catabolites of glucose activate the HPr kinase, and then the phosphorylated form of HPr(Ser) binds to CcpA, mediating the dimerization of CcpA ( 12,  34,  37).	bind
16547	2	5521	6	10	NULL	NULL	NULL	HPr	GP	phosphorylated	bind			Ser		CcpA	GP				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_64_7_2513_s_193	9647823	(i) Catabolites of glucose activate the HPr kinase, and then the phosphorylated form of HPr(Ser) binds to CcpA, mediating the dimerization of CcpA ( 12,  34,  37).	bind
16548	3	5521	6	10	NULL	NULL	NULL	statement 2	Process		mediates					CcpA	GP	dimerization of			NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_64_7_2513_s_193	9647823	(i) Catabolites of glucose activate the HPr kinase, and then the phosphorylated form of HPr(Ser) binds to CcpA, mediating the dimerization of CcpA ( 12,  34,  37).	bind
15811	1	5521	7	10	NULL	NULL	NULL	glucose catabolites	Chemical		activates					HPr kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_64_7_2513_s_193	9647823	(i) Catabolites of glucose activate the HPr kinase, and then the phosphorylated form of HPr(Ser) binds to CcpA, mediating the dimerization of CcpA ( 12,  34,  37).	bind
15812	2	5521	7	10	NULL	NULL	NULL	HPr	GP	phosphorylated	bind			Ser		CcpA	GP				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_64_7_2513_s_193	9647823	(i) Catabolites of glucose activate the HPr kinase, and then the phosphorylated form of HPr(Ser) binds to CcpA, mediating the dimerization of CcpA ( 12,  34,  37).	bind
15813	3	5521	7	10	NULL	NULL	NULL	statement 2	Process		mediates					CcpA	GP	dimerization of			NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_64_7_2513_s_193	9647823	(i) Catabolites of glucose activate the HPr kinase, and then the phosphorylated form of HPr(Ser) binds to CcpA, mediating the dimerization of CcpA ( 12,  34,  37).	bind
16549	1	5522	6	10	NULL	NULL	NULL	CcpA	GP		bind		efficiently			phoPR	GP			CRE site of promoter	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbacteriol_188_4_1266_s_296	16452408	(i) CcpA without cofactors binds efficiently to the  phoPR promoter  cre site ( Kd  0.5 nM) but required more than 1 muM CcpA to inhibit PA6 transcription in vitro in the absence of coeffectors.	bind
16550	2	5522	6	10	NULL	NULL	NULL	CcpA	GP		inhibit					PA6	GP	transcription of			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbacteriol_188_4_1266_s_296	16452408	(i) CcpA without cofactors binds efficiently to the  phoPR promoter  cre site ( Kd  0.5 nM) but required more than 1 muM CcpA to inhibit PA6 transcription in vitro in the absence of coeffectors.	bind
16551	3	5522	6	10	NULL	NULL	NULL	statement 2	Process		occurs in absence of					coeffectors	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbacteriol_188_4_1266_s_296	16452408	(i) CcpA without cofactors binds efficiently to the  phoPR promoter  cre site ( Kd  0.5 nM) but required more than 1 muM CcpA to inhibit PA6 transcription in vitro in the absence of coeffectors.	bind
53105	4	5522	6	10	NULL	NULL	NULL	statement 1	Process		occurs without					CcpA	GP	cofactors of			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbacteriol_188_4_1266_s_296	16452408	(i) CcpA without cofactors binds efficiently to the  phoPR promoter  cre site ( Kd  0.5 nM) but required more than 1 muM CcpA to inhibit PA6 transcription in vitro in the absence of coeffectors.	bind
15814	1	5522	7	10	NULL	NULL	NULL	CcpA	GP		binds		efficiently			 phoPR	GP			promoter cre site	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbacteriol_188_4_1266_s_296	16452408	(i) CcpA without cofactors binds efficiently to the  phoPR promoter  cre site ( Kd  0.5 nM) but required more than 1 muM CcpA to inhibit PA6 transcription in vitro in the absence of coeffectors.	bind
15815	2	5522	7	10	NULL	NULL	NULL	statement 1	Process		occur without					CcpA	GP	cofactors of			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbacteriol_188_4_1266_s_296	16452408	(i) CcpA without cofactors binds efficiently to the  phoPR promoter  cre site ( Kd  0.5 nM) but required more than 1 muM CcpA to inhibit PA6 transcription in vitro in the absence of coeffectors.	bind
15816	3	5522	7	10	NULL	NULL	NULL	CcpA	GP		inhibit					PA6	GP	transcription of			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbacteriol_188_4_1266_s_296	16452408	(i) CcpA without cofactors binds efficiently to the  phoPR promoter  cre site ( Kd  0.5 nM) but required more than 1 muM CcpA to inhibit PA6 transcription in vitro in the absence of coeffectors.	bind
15817	4	5522	7	10	NULL	NULL	NULL	statement 3	Process		occurs in the absence of					coeffectors	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbacteriol_188_4_1266_s_296	16452408	(i) CcpA without cofactors binds efficiently to the  phoPR promoter  cre site ( Kd  0.5 nM) but required more than 1 muM CcpA to inhibit PA6 transcription in vitro in the absence of coeffectors.	bind
16552	1	5523	6	10	NULL	NULL	NULL	E.coli	Organism		bind					CHO cells	Cell	SR-A transfected			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_4_1953_s_119	10722588	(i) Characteristics of binding of  E. coli by SR-A-transfected CHO cells.	bind
15818	1	5523	7	10	NULL	NULL	NULL	E.coli	Organism		bind					CHO cells	Cell	SR-A-transfected			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_4_1953_s_119	10722588	(i) Characteristics of binding of  E. coli by SR-A-transfected CHO cells.	bind
16756	1	5524	6	10	NULL	NULL	NULL	PU.1	GP		associates with					GATA-1 target gene	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7460_s_372	14559995	(i) ChIP experiments indicate that PU.1 and pRB can be found associated with a GATA-1 target gene, but only when both GATA-1 and an intact GATA-1 DNA binding site are present.	bind
16757	2	5524	6	10	NULL	NULL	NULL	pRB	GP		associates with					GATA-1 target gene	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7460_s_372	14559995	(i) ChIP experiments indicate that PU.1 and pRB can be found associated with a GATA-1 target gene, but only when both GATA-1 and an intact GATA-1 DNA binding site are present.	bind
16760	3	5524	6	10	NULL	NULL	NULL	statement 1	Process		occurs in presence of		only					intact		GATA-1 DNA binding site	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7460_s_372	14559995	(i) ChIP experiments indicate that PU.1 and pRB can be found associated with a GATA-1 target gene, but only when both GATA-1 and an intact GATA-1 DNA binding site are present.	bind
16761	4	5524	6	10	NULL	NULL	NULL	statement 1	Process		occurs in presence of		only			GATA-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7460_s_372	14559995	(i) ChIP experiments indicate that PU.1 and pRB can be found associated with a GATA-1 target gene, but only when both GATA-1 and an intact GATA-1 DNA binding site are present.	bind
17044	5	5524	6	10	NULL	NULL	NULL	statement 3	Process		occurs simultaneously with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7460_s_372	14559995	(i) ChIP experiments indicate that PU.1 and pRB can be found associated with a GATA-1 target gene, but only when both GATA-1 and an intact GATA-1 DNA binding site are present.	bind
17045	6	5524	6	10	NULL	NULL	NULL	statement 2	Process		occurs in presence of		only					intact		GATA-1 DNA binding site	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7460_s_372	14559995	(i) ChIP experiments indicate that PU.1 and pRB can be found associated with a GATA-1 target gene, but only when both GATA-1 and an intact GATA-1 DNA binding site are present.	bind
17046	7	5524	6	10	NULL	NULL	NULL	statement 2	Process		occurs in presence of		only			GATA-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7460_s_372	14559995	(i) ChIP experiments indicate that PU.1 and pRB can be found associated with a GATA-1 target gene, but only when both GATA-1 and an intact GATA-1 DNA binding site are present.	bind
17047	8	5524	6	10	NULL	NULL	NULL	statement 6	Process		occurs simultaneously with					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7460_s_372	14559995	(i) ChIP experiments indicate that PU.1 and pRB can be found associated with a GATA-1 target gene, but only when both GATA-1 and an intact GATA-1 DNA binding site are present.	bind
15819	1	5524	7	10	NULL	NULL	NULL	PU.1	GP		associate with					GATA-1 target gene	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7460_s_372	14559995	(i) ChIP experiments indicate that PU.1 and pRB can be found associated with a GATA-1 target gene, but only when both GATA-1 and an intact GATA-1 DNA binding site are present.	bind
15820	2	5524	7	10	NULL	NULL	NULL	pRB	GP		associate with					GATA-1 target gene	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7460_s_372	14559995	(i) ChIP experiments indicate that PU.1 and pRB can be found associated with a GATA-1 target gene, but only when both GATA-1 and an intact GATA-1 DNA binding site are present.	bind
15821	3	5524	7	10	NULL	NULL	NULL	statement 1	Process		occurs in the presence of		only			GATA-1 	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7460_s_372	14559995	(i) ChIP experiments indicate that PU.1 and pRB can be found associated with a GATA-1 target gene, but only when both GATA-1 and an intact GATA-1 DNA binding site are present.	bind
15822	4	5524	7	10	NULL	NULL	NULL	statement 2	Process		occurs in the presence of		only			GATA-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7460_s_372	14559995	(i) ChIP experiments indicate that PU.1 and pRB can be found associated with a GATA-1 target gene, but only when both GATA-1 and an intact GATA-1 DNA binding site are present.	bind
15823	5	5524	7	10	NULL	NULL	NULL	statement 1	Process		occurs in the presence of		only					intact		GATA-1 DNA binding site	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7460_s_372	14559995	(i) ChIP experiments indicate that PU.1 and pRB can be found associated with a GATA-1 target gene, but only when both GATA-1 and an intact GATA-1 DNA binding site are present.	bind
15824	6	5524	7	10	NULL	NULL	NULL	statement 2	Process		occurs in the presence of		only					intact		GATA-1 DNA binding site	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7460_s_372	14559995	(i) ChIP experiments indicate that PU.1 and pRB can be found associated with a GATA-1 target gene, but only when both GATA-1 and an intact GATA-1 DNA binding site are present.	bind
15825	7	5524	7	10	NULL	NULL	NULL	statement 3	Process		occurs simultaneous with					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7460_s_372	14559995	(i) ChIP experiments indicate that PU.1 and pRB can be found associated with a GATA-1 target gene, but only when both GATA-1 and an intact GATA-1 DNA binding site are present.	bind
15826	8	5524	7	10	NULL	NULL	NULL	statement 4	Process		occurs simultaneous with					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7460_s_372	14559995	(i) ChIP experiments indicate that PU.1 and pRB can be found associated with a GATA-1 target gene, but only when both GATA-1 and an intact GATA-1 DNA binding site are present.	bind
16553	1	5525	6	10	NULL	NULL	NULL	uracil	Chemical		bind					UDGs	GP		active site pocket		NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_24_7216_s_188	14654697	(i) Co-crystal structures of uracil and UDG have shown that at least one site of uracil binding to UDGs is the active site pocket ( 14, 15).	bind
15827	1	5525	7	10	NULL	NULL	NULL	uracil	Chemical		bind					UDGs	GP		active site pocket		NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_24_7216_s_188	14654697	(i) Co-crystal structures of uracil and UDG have shown that at least one site of uracil binding to UDGs is the active site pocket ( 14, 15).	bind
16554	1	5526	6	10	NULL	NULL	NULL	Coagulation factor G	GP		bind					beta-1,3-glucans	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_38_24948_s_233	9733802	(i) Coagulation factor G binds beta-1,3-glucans but not LPS ( 43).	bind
16555	2	5526	6	10	NULL	NULL	NULL	Coagulation factor G	GP		does not bind					LPS	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_38_24948_s_233	9733802	(i) Coagulation factor G binds beta-1,3-glucans but not LPS ( 43).	bind
15832	1	5526	7	10	NULL	NULL	NULL	Coagulation factor G	GP		binds					beta-1,3-glucans	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_38_24948_s_233	9733802	(i) Coagulation factor G binds beta-1,3-glucans but not LPS ( 43).	bind
15833	2	5526	7	10	NULL	NULL	NULL	Coagulation factor G	GP		does not bind					LPS	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_38_24948_s_233	9733802	(i) Coagulation factor G binds beta-1,3-glucans but not LPS ( 43).	bind
16556	1	5527	6	10	NULL	NULL	NULL	collagen cDNA	NucleicAcid		bind		specifically			alpha1	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_17_12475_s_48	10777533	(I) collagen cDNA that specifically binds human alpha1	bind
15834	1	5527	7	10	NULL	NULL	NULL	collagen cDNA	NucleicAcid		binds		specifically			alpha1	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_17_12475_s_48	10777533	(I) collagen cDNA that specifically binds human alpha1	bind
16557	1	5528	6	10	NULL	NULL	NULL	decorin	GP		bind					collagen	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_29_21801_s_60	10823816	(I) Collagen Chain-- Binding of decorin to collagen interferes with horizontal accretion of collagen molecules and prevents lateral growth of the fibrils ( 2).	bind
16558	2	5528	6	10	NULL	NULL	NULL	statement 1	Process		interferes with					collagen molecules	GP	horizontal accretion of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_29_21801_s_60	10823816	(I) Collagen Chain-- Binding of decorin to collagen interferes with horizontal accretion of collagen molecules and prevents lateral growth of the fibrils ( 2).	bind
16559	3	5528	6	10	NULL	NULL	NULL	statement 1	Process		prevents					fibrils	OrganismPart	lateral growth of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_29_21801_s_60	10823816	(I) Collagen Chain-- Binding of decorin to collagen interferes with horizontal accretion of collagen molecules and prevents lateral growth of the fibrils ( 2).	bind
15835	1	5528	7	10	NULL	NULL	NULL	decorin	GP		binds					collagen	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_29_21801_s_60	10823816	(I) Collagen Chain-- Binding of decorin to collagen interferes with horizontal accretion of collagen molecules and prevents lateral growth of the fibrils ( 2).	bind
15836	2	5528	7	10	NULL	NULL	NULL	statement 1	Process		interferes with					collagen molecules	GP	horizontal accretion of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_29_21801_s_60	10823816	(I) Collagen Chain-- Binding of decorin to collagen interferes with horizontal accretion of collagen molecules and prevents lateral growth of the fibrils ( 2).	bind
15837	3	5528	7	10	NULL	NULL	NULL	statement 2	Process		prevents					fibrils	OrganismPart	lateral growth of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_29_21801_s_60	10823816	(I) Collagen Chain-- Binding of decorin to collagen interferes with horizontal accretion of collagen molecules and prevents lateral growth of the fibrils ( 2).	bind
16560	1	5529	6	10	NULL	NULL	NULL	BTEB	GP		is					basic transcription element binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2818_s_57	10733585	(I) collagen gene, and the GC box was bound by a DNA binding protein, termed BTEB (basic transcription element binding protein) ( 8).	bind
16561	2	5529	6	10	NULL	NULL	NULL	BTEB	GP		bind					collagen gene	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2818_s_57	10733585	(I) collagen gene, and the GC box was bound by a DNA binding protein, termed BTEB (basic transcription element binding protein) ( 8).	bind
16562	3	5529	6	10	NULL	NULL	NULL	BTEB	GP		bind									GC box	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2818_s_57	10733585	(I) collagen gene, and the GC box was bound by a DNA binding protein, termed BTEB (basic transcription element binding protein) ( 8).	bind
44808	4	5529	6	10	NULL	NULL	NULL	BTEB	GP		is a type of					DNA binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2818_s_57	10733585	(I) collagen gene, and the GC box was bound by a DNA binding protein, termed BTEB (basic transcription element binding protein) ( 8).	bind
15838	1	5529	7	10	NULL	NULL	NULL	BTEB	GP		bind					collagen gene	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2818_s_57	10733585	(I) collagen gene, and the GC box was bound by a DNA binding protein, termed BTEB (basic transcription element binding protein) ( 8).	bind
15839	2	5529	7	10	NULL	NULL	NULL	BTEB	GP		binds									GC box	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2818_s_57	10733585	(I) collagen gene, and the GC box was bound by a DNA binding protein, termed BTEB (basic transcription element binding protein) ( 8).	bind
15840	3	5529	7	10	NULL	NULL	NULL	BTEB	GP		is					basic transcription element binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2818_s_57	10733585	(I) collagen gene, and the GC box was bound by a DNA binding protein, termed BTEB (basic transcription element binding protein) ( 8).	bind
15841	4	5529	7	10	NULL	NULL	NULL	BTEB	GP		is a type of					DNA binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2818_s_57	10733585	(I) collagen gene, and the GC box was bound by a DNA binding protein, termed BTEB (basic transcription element binding protein) ( 8).	bind
16563	1	5531	6	10	NULL	NULL	NULL	HMG-I(Y)	GP		modulates					NF-Y function	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_49_30880_s_29	9388234	(I) collagen promoter and multimerized version of the alpha2(I) collagen NF-Y(CBF) binding site have been used to investigate the role of HMG-I(Y) as a protein cofactor in modulating NF-Y function.	bind
16564	2	5531	6	10	NULL	NULL	NULL	HMG-I(Y)	GP		is a type of					protien cofactor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_49_30880_s_29	9388234	(I) collagen promoter and multimerized version of the alpha2(I) collagen NF-Y(CBF) binding site have been used to investigate the role of HMG-I(Y) as a protein cofactor in modulating NF-Y function.	bind
20334	1	5531	7	10	NULL	NULL	NULL	HMG-I(Y)	GP		modulates					NF-Y function	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_49_30880_s_29	9388234	(I) collagen promoter and multimerized version of the alpha2(I) collagen NF-Y(CBF) binding site have been used to investigate the role of HMG-I(Y) as a protein cofactor in modulating NF-Y function.	bind
20335	2	5531	7	10	NULL	NULL	NULL	HMG-I(Y)	GP		is a type of					protein cofactor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_49_30880_s_29	9388234	(I) collagen promoter and multimerized version of the alpha2(I) collagen NF-Y(CBF) binding site have been used to investigate the role of HMG-I(Y) as a protein cofactor in modulating NF-Y function.	bind
16565	1	5532	6	10	NULL	NULL	NULL	NF-Y	GP		bind					cell-cycle genes	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_33_30435_s_136	12771133	(i) Contrary to predictions based upon  in  vitro binding activity in EMSAs and ChIP data on other promoters, the   in vivo binding of NF-Y to cell-cycle genes is strictly regulated  during the different phases of the cell-cycle.	bind
16566	2	5532	6	10	NULL	NULL	NULL	statement 1	Process		is regulated during		strictly			cell cycle	Process	different phases of 			NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_33_30435_s_136	12771133	(i) Contrary to predictions based upon  in  vitro binding activity in EMSAs and ChIP data on other promoters, the   in vivo binding of NF-Y to cell-cycle genes is strictly regulated  during the different phases of the cell-cycle.	bind
15842	1	5532	7	10	NULL	NULL	NULL	NF-Y	GP		bind					cell-cycle genes	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_33_30435_s_136	12771133	(i) Contrary to predictions based upon  in  vitro binding activity in EMSAs and ChIP data on other promoters, the   in vivo binding of NF-Y to cell-cycle genes is strictly regulated  during the different phases of the cell-cycle.	bind
15843	2	5532	7	10	NULL	NULL	NULL	statement 1	Process		is regulated during		strictly			cell-cycle	Process	different phases of			NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_33_30435_s_136	12771133	(i) Contrary to predictions based upon  in  vitro binding activity in EMSAs and ChIP data on other promoters, the   in vivo binding of NF-Y to cell-cycle genes is strictly regulated  during the different phases of the cell-cycle.	bind
16837	1	5533	6	NULL	NULL	0	NULL		NULL		bind	NULL	directly	region I			NULL		region II		NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_4_1414_s_268	16449652	(i) Direct interactions  between regions I and II are important for masking the NLS, and the signal-dependent  binding of unknown factor "`X"` to the region spanning aa residues 183 to  382 disrupts this masking.	bind
16839	2	5533	6	10	NULL	NULL	NULL	statement 1	Process		is important for					NLS	GP	masking of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_4_1414_s_268	16449652	(i) Direct interactions  between regions I and II are important for masking the NLS, and the signal-dependent  binding of unknown factor "`X"` to the region spanning aa residues 183 to  382 disrupts this masking.	bind
16840	3	5533	6	10	NULL	NULL	NULL	unknown factor X	GP		bind								aa residues 183 to 382		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_4_1414_s_268	16449652	(i) Direct interactions  between regions I and II are important for masking the NLS, and the signal-dependent  binding of unknown factor "`X"` to the region spanning aa residues 183 to  382 disrupts this masking.	bind
16841	4	5533	6	10	NULL	NULL	NULL	statement 3	Process		is dependent on					signal	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_4_1414_s_268	16449652	(i) Direct interactions  between regions I and II are important for masking the NLS, and the signal-dependent  binding of unknown factor "`X"` to the region spanning aa residues 183 to  382 disrupts this masking.	bind
16842	5	5533	6	10	NULL	NULL	NULL	statement 4	Process		disrupts					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_4_1414_s_268	16449652	(i) Direct interactions  between regions I and II are important for masking the NLS, and the signal-dependent  binding of unknown factor "`X"` to the region spanning aa residues 183 to  382 disrupts this masking.	bind
15844	1	5533	7	NULL	NULL	0	NULL		NULL		bind	NULL	directly	region I			NULL		region II		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_4_1414_s_268	16449652	(i) Direct interactions  between regions I and II are important for masking the NLS, and the signal-dependent  binding of unknown factor "`X"` to the region spanning aa residues 183 to  382 disrupts this masking.	bind
15845	2	5533	7	10	NULL	NULL	NULL	statement 1	Process		is important for					NLS	GP	masking			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_4_1414_s_268	16449652	(i) Direct interactions  between regions I and II are important for masking the NLS, and the signal-dependent  binding of unknown factor "`X"` to the region spanning aa residues 183 to  382 disrupts this masking.	bind
15846	3	5533	7	10	NULL	NULL	NULL	unknown factor X	GP		binds								region spanning aa residues 183 to 382 		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_4_1414_s_268	16449652	(i) Direct interactions  between regions I and II are important for masking the NLS, and the signal-dependent  binding of unknown factor "`X"` to the region spanning aa residues 183 to  382 disrupts this masking.	bind
15847	4	5533	7	10	NULL	NULL	NULL	statement 3	Process		is dependent on					signal	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_4_1414_s_268	16449652	(i) Direct interactions  between regions I and II are important for masking the NLS, and the signal-dependent  binding of unknown factor "`X"` to the region spanning aa residues 183 to  382 disrupts this masking.	bind
15848	5	5533	7	10	NULL	NULL	NULL	statement 3	Process		disrupts					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_4_1414_s_268	16449652	(i) Direct interactions  between regions I and II are important for masking the NLS, and the signal-dependent  binding of unknown factor "`X"` to the region spanning aa residues 183 to  382 disrupts this masking.	bind
16567	1	5535	6	10	NULL	NULL	NULL	MAb FRP5	GP		activates					ErbB-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5042_s_322	9710588	(i) ErbB-2 activated by MAb FRP5 and ErbB-2 activated by NDF displayed similar levels of total phosphotyrosine; however, GST-Grb2 SH2 bound significantly higher amounts of FRP5-activated ErbB-2.	bind
16568	2	5535	6	10	NULL	NULL	NULL	NDF	GP		activates					ErbB-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5042_s_322	9710588	(i) ErbB-2 activated by MAb FRP5 and ErbB-2 activated by NDF displayed similar levels of total phosphotyrosine; however, GST-Grb2 SH2 bound significantly higher amounts of FRP5-activated ErbB-2.	bind
16569	3	5535	6	10	NULL	NULL	NULL	FRP5	GP		activates					ErbB-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5042_s_322	9710588	(i) ErbB-2 activated by MAb FRP5 and ErbB-2 activated by NDF displayed similar levels of total phosphotyrosine; however, GST-Grb2 SH2 bound significantly higher amounts of FRP5-activated ErbB-2.	bind
16570	4	5535	6	10	NULL	NULL	NULL	GST-Grb2	GP		bind		significantly	SH2 domain		ErB-2	GP	FRP5 activated			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5042_s_322	9710588	(i) ErbB-2 activated by MAb FRP5 and ErbB-2 activated by NDF displayed similar levels of total phosphotyrosine; however, GST-Grb2 SH2 bound significantly higher amounts of FRP5-activated ErbB-2.	bind
15849	1	5535	7	10	NULL	NULL	NULL	MAb FRP5	GP		activates					ErbB-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5042_s_322	9710588	(i) ErbB-2 activated by MAb FRP5 and ErbB-2 activated by NDF displayed similar levels of total phosphotyrosine; however, GST-Grb2 SH2 bound significantly higher amounts of FRP5-activated ErbB-2.	bind
15850	2	5535	7	10	NULL	NULL	NULL	NDF	GP		activates					ErbB-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5042_s_322	9710588	(i) ErbB-2 activated by MAb FRP5 and ErbB-2 activated by NDF displayed similar levels of total phosphotyrosine; however, GST-Grb2 SH2 bound significantly higher amounts of FRP5-activated ErbB-2.	bind
15851	3	5535	7	10	NULL	NULL	NULL	statement 1	Process	levels of total	is similar to			phosphotyrosine		statement 2	Process	levels of total	phosphotyrosine		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5042_s_322	9710588	(i) ErbB-2 activated by MAb FRP5 and ErbB-2 activated by NDF displayed similar levels of total phosphotyrosine; however, GST-Grb2 SH2 bound significantly higher amounts of FRP5-activated ErbB-2.	bind
15852	4	5535	7	10	NULL	NULL	NULL	FRP5	GP		activates					ErbB-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5042_s_322	9710588	(i) ErbB-2 activated by MAb FRP5 and ErbB-2 activated by NDF displayed similar levels of total phosphotyrosine; however, GST-Grb2 SH2 bound significantly higher amounts of FRP5-activated ErbB-2.	bind
15853	5	5535	7	10	NULL	NULL	NULL	GST-Grb2	GP		bind		significantly	SH2		ErbB-2	GP	FRP5-activated 			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5042_s_322	9710588	(i) ErbB-2 activated by MAb FRP5 and ErbB-2 activated by NDF displayed similar levels of total phosphotyrosine; however, GST-Grb2 SH2 bound significantly higher amounts of FRP5-activated ErbB-2.	bind
16749	1	5538	6	10	NULL	NULL	NULL	substrate protein	GP		loaded into					GroEL	GP		heptamer ring		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45737_s_18	15347650	(i) For  cis-ternary complex formation, the binding of ATP to the substrate protein-loaded heptamer ring of GroEL permits the binding of GroES to this ring ( cis-ring) generating an enlarged, closed central cavity ( cis-cavity) in which the substrate protein is discharged ( cis-ATP complex) ( ).	bind
16751	2	5538	6	10	NULL	NULL	NULL	ATP	Chemical		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45737_s_18	15347650	(i) For  cis-ternary complex formation, the binding of ATP to the substrate protein-loaded heptamer ring of GroEL permits the binding of GroES to this ring ( cis-ring) generating an enlarged, closed central cavity ( cis-cavity) in which the substrate protein is discharged ( cis-ATP complex) ( ).	bind
16752	3	5538	6	10	NULL	NULL	NULL	GroES	GP		bind					GroEL	GP		heptamer ring		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45737_s_18	15347650	(i) For  cis-ternary complex formation, the binding of ATP to the substrate protein-loaded heptamer ring of GroEL permits the binding of GroES to this ring ( cis-ring) generating an enlarged, closed central cavity ( cis-cavity) in which the substrate protein is discharged ( cis-ATP complex) ( ).	bind
16754	4	5538	6	10	NULL	NULL	NULL	statement 2	Process		permits					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45737_s_18	15347650	(i) For  cis-ternary complex formation, the binding of ATP to the substrate protein-loaded heptamer ring of GroEL permits the binding of GroES to this ring ( cis-ring) generating an enlarged, closed central cavity ( cis-cavity) in which the substrate protein is discharged ( cis-ATP complex) ( ).	bind
44823	5	5538	6	10	NULL	NULL	NULL	statement 3	Process		generates					cis-cavity					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45737_s_18	15347650	(i) For  cis-ternary complex formation, the binding of ATP to the substrate protein-loaded heptamer ring of GroEL permits the binding of GroES to this ring ( cis-ring) generating an enlarged, closed central cavity ( cis-cavity) in which the substrate protein is discharged ( cis-ATP complex) ( ).	bind
44824	6	5538	6	10	NULL	NULL	NULL	substrate protein	GP		is discharged into					cis-cavity					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45737_s_18	15347650	(i) For  cis-ternary complex formation, the binding of ATP to the substrate protein-loaded heptamer ring of GroEL permits the binding of GroES to this ring ( cis-ring) generating an enlarged, closed central cavity ( cis-cavity) in which the substrate protein is discharged ( cis-ATP complex) ( ).	bind
44825	7	5538	6	10	NULL	0	NULL	cis-cavity	NULL		is an	NULL				closed central cavity	NULL	enlarged			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_44_45737_s_18	15347650	(i) For  cis-ternary complex formation, the binding of ATP to the substrate protein-loaded heptamer ring of GroEL permits the binding of GroES to this ring ( cis-ring) generating an enlarged, closed central cavity ( cis-cavity) in which the substrate protein is discharged ( cis-ATP complex) ( ).	bind
44826	8	5538	6	10	NULL	NULL	NULL	cis-ternary complex	GP	formation of	involves					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45737_s_18	15347650	(i) For  cis-ternary complex formation, the binding of ATP to the substrate protein-loaded heptamer ring of GroEL permits the binding of GroES to this ring ( cis-ring) generating an enlarged, closed central cavity ( cis-cavity) in which the substrate protein is discharged ( cis-ATP complex) ( ).	bind
15886	1	5538	7	10	NULL	NULL	NULL	substrate protein	GP		is loaded with					GroEL	GP		heptamer ring 		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45737_s_18	15347650	(i) For  cis-ternary complex formation, the binding of ATP to the substrate protein-loaded heptamer ring of GroEL permits the binding of GroES to this ring ( cis-ring) generating an enlarged, closed central cavity ( cis-cavity) in which the substrate protein is discharged ( cis-ATP complex) ( ).	bind
15887	2	5538	7	10	NULL	NULL	NULL	ATP	Chemical		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45737_s_18	15347650	(i) For  cis-ternary complex formation, the binding of ATP to the substrate protein-loaded heptamer ring of GroEL permits the binding of GroES to this ring ( cis-ring) generating an enlarged, closed central cavity ( cis-cavity) in which the substrate protein is discharged ( cis-ATP complex) ( ).	bind
15889	3	5538	7	10	NULL	NULL	NULL	GroES	GP		bind					GroEL	GP	 	cis- ring		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45737_s_18	15347650	(i) For  cis-ternary complex formation, the binding of ATP to the substrate protein-loaded heptamer ring of GroEL permits the binding of GroES to this ring ( cis-ring) generating an enlarged, closed central cavity ( cis-cavity) in which the substrate protein is discharged ( cis-ATP complex) ( ).	bind
15893	4	5538	7	10	NULL	NULL	NULL	statement 2	Process		permits					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45737_s_18	15347650	(i) For  cis-ternary complex formation, the binding of ATP to the substrate protein-loaded heptamer ring of GroEL permits the binding of GroES to this ring ( cis-ring) generating an enlarged, closed central cavity ( cis-cavity) in which the substrate protein is discharged ( cis-ATP complex) ( ).	bind
15898	5	5538	7	10	NULL	NULL	NULL	statement 3	Process		generates					cis-cavity					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45737_s_18	15347650	(i) For  cis-ternary complex formation, the binding of ATP to the substrate protein-loaded heptamer ring of GroEL permits the binding of GroES to this ring ( cis-ring) generating an enlarged, closed central cavity ( cis-cavity) in which the substrate protein is discharged ( cis-ATP complex) ( ).	bind
15901	6	5538	7	10	NULL	NULL	NULL	substrate protein	GP		is discharged into					cis-cavity					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45737_s_18	15347650	(i) For  cis-ternary complex formation, the binding of ATP to the substrate protein-loaded heptamer ring of GroEL permits the binding of GroES to this ring ( cis-ring) generating an enlarged, closed central cavity ( cis-cavity) in which the substrate protein is discharged ( cis-ATP complex) ( ).	bind
15904	7	5538	7	NULL	NULL	0	NULL	cis-cavity	NULL		is an	NULL				closed central cavity	NULL	enlarged			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_44_45737_s_18	15347650	(i) For  cis-ternary complex formation, the binding of ATP to the substrate protein-loaded heptamer ring of GroEL permits the binding of GroES to this ring ( cis-ring) generating an enlarged, closed central cavity ( cis-cavity) in which the substrate protein is discharged ( cis-ATP complex) ( ).	bind
15908	8	5538	7	10	NULL	NULL	NULL	cis-ternary complex 	GP	formation of	involves					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45737_s_18	15347650	(i) For  cis-ternary complex formation, the binding of ATP to the substrate protein-loaded heptamer ring of GroEL permits the binding of GroES to this ring ( cis-ring) generating an enlarged, closed central cavity ( cis-cavity) in which the substrate protein is discharged ( cis-ATP complex) ( ).	bind
16571	1	5539	6	10	NULL	NULL	NULL	fVIII	GP		bind					LRP	GP	purified			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_53_37685_s_249	10608826	(i) fVIII binds to purified LRP with the affinity similar (within 2-fold) to that determined in our study.	bind
15909	1	5539	7	10	NULL	NULL	NULL	fVIII	GP		bind					LRP	GP	purified			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_53_37685_s_249	10608826	(i) fVIII binds to purified LRP with the affinity similar (within 2-fold) to that determined in our study.	bind
16734	1	5540	6	10	NULL	NULL	NULL	Galectin-1	GP		is found in					cytosol	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_10_5198_s_18	7890630	(i) Galectin-1 is found  mainly in the cytosol of most cells in which it occurs (Briles  et  al., 1979), (ii) the lectin has free sulfhydryls and is inactive  in the absence of reducing agents (Hirabayashi and Kasai, 1991;  Barondes, 1984), (iii) the lectin lacks an identifiable signal sequence  and does not appear to be secreted through the normal secretory pathway  in differentiated myoblasts (Cooper and Barondes, 1990), (iv) the  lectin binds to beta-galactosyl-containing glycoconjugates on the cell  surface and in the extracellular matrix (Cerra  et al., 1984;  Merkle and Cummings, 1988;	bind
16735	2	5540	6	10	NULL	NULL	NULL	lectin	GP		bind					beta-galactosyl-containing glycoconjugates	Chemical				NULL	cell surface	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_10_5198_s_18	7890630	(i) Galectin-1 is found  mainly in the cytosol of most cells in which it occurs (Briles  et  al., 1979), (ii) the lectin has free sulfhydryls and is inactive  in the absence of reducing agents (Hirabayashi and Kasai, 1991;  Barondes, 1984), (iii) the lectin lacks an identifiable signal sequence  and does not appear to be secreted through the normal secretory pathway  in differentiated myoblasts (Cooper and Barondes, 1990), (iv) the  lectin binds to beta-galactosyl-containing glycoconjugates on the cell  surface and in the extracellular matrix (Cerra  et al., 1984;  Merkle and Cummings, 1988;	bind
16736	3	5540	6	10	NULL	NULL	NULL	lectin	GP		bind					beta-galactosyl-containing glycoconjugates	Chemical				NULL	extracellular matrix	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_10_5198_s_18	7890630	(i) Galectin-1 is found  mainly in the cytosol of most cells in which it occurs (Briles  et  al., 1979), (ii) the lectin has free sulfhydryls and is inactive  in the absence of reducing agents (Hirabayashi and Kasai, 1991;  Barondes, 1984), (iii) the lectin lacks an identifiable signal sequence  and does not appear to be secreted through the normal secretory pathway  in differentiated myoblasts (Cooper and Barondes, 1990), (iv) the  lectin binds to beta-galactosyl-containing glycoconjugates on the cell  surface and in the extracellular matrix (Cerra  et al., 1984;  Merkle and Cummings, 1988;	bind
16738	4	5540	6	10	NULL	NULL	NULL	lectin	GP		is inactive					reducing agents	Chemical	in absence of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_10_5198_s_18	7890630	(i) Galectin-1 is found  mainly in the cytosol of most cells in which it occurs (Briles  et  al., 1979), (ii) the lectin has free sulfhydryls and is inactive  in the absence of reducing agents (Hirabayashi and Kasai, 1991;  Barondes, 1984), (iii) the lectin lacks an identifiable signal sequence  and does not appear to be secreted through the normal secretory pathway  in differentiated myoblasts (Cooper and Barondes, 1990), (iv) the  lectin binds to beta-galactosyl-containing glycoconjugates on the cell  surface and in the extracellular matrix (Cerra  et al., 1984;  Merkle and Cummings, 1988;	bind
16739	5	5540	6	10	NULL	NULL	NULL	lectin	GP		is not secreted through					secretory pathway	Process	normal			NULL	differentiated myoblasts	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_10_5198_s_18	7890630	(i) Galectin-1 is found  mainly in the cytosol of most cells in which it occurs (Briles  et  al., 1979), (ii) the lectin has free sulfhydryls and is inactive  in the absence of reducing agents (Hirabayashi and Kasai, 1991;  Barondes, 1984), (iii) the lectin lacks an identifiable signal sequence  and does not appear to be secreted through the normal secretory pathway  in differentiated myoblasts (Cooper and Barondes, 1990), (iv) the  lectin binds to beta-galactosyl-containing glycoconjugates on the cell  surface and in the extracellular matrix (Cerra  et al., 1984;  Merkle and Cummings, 1988;	bind
16743	6	5540	6	10	NULL	NULL	NULL	lectin	GP		lacks an							identifiable		signal sequence	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_10_5198_s_18	7890630	(i) Galectin-1 is found  mainly in the cytosol of most cells in which it occurs (Briles  et  al., 1979), (ii) the lectin has free sulfhydryls and is inactive  in the absence of reducing agents (Hirabayashi and Kasai, 1991;  Barondes, 1984), (iii) the lectin lacks an identifiable signal sequence  and does not appear to be secreted through the normal secretory pathway  in differentiated myoblasts (Cooper and Barondes, 1990), (iv) the  lectin binds to beta-galactosyl-containing glycoconjugates on the cell  surface and in the extracellular matrix (Cerra  et al., 1984;  Merkle and Cummings, 1988;	bind
15924	1	5540	7	10	NULL	NULL	NULL	Galectin-1	GP		is found in					cytosol	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_10_5198_s_18	7890630	(i) Galectin-1 is found  mainly in the cytosol of most cells in which it occurs (Briles  et  al., 1979), (ii) the lectin has free sulfhydryls and is inactive  in the absence of reducing agents (Hirabayashi and Kasai, 1991;  Barondes, 1984), (iii) the lectin lacks an identifiable signal sequence  and does not appear to be secreted through the normal secretory pathway  in differentiated myoblasts (Cooper and Barondes, 1990), (iv) the  lectin binds to beta-galactosyl-containing glycoconjugates on the cell  surface and in the extracellular matrix (Cerra  et al., 1984;  Merkle and Cummings, 1988;	bind
15930	2	5540	7	10	NULL	NULL	NULL	Lectin	GP		contains					sulfhydryls	Chemical	free			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_10_5198_s_18	7890630	(i) Galectin-1 is found  mainly in the cytosol of most cells in which it occurs (Briles  et  al., 1979), (ii) the lectin has free sulfhydryls and is inactive  in the absence of reducing agents (Hirabayashi and Kasai, 1991;  Barondes, 1984), (iii) the lectin lacks an identifiable signal sequence  and does not appear to be secreted through the normal secretory pathway  in differentiated myoblasts (Cooper and Barondes, 1990), (iv) the  lectin binds to beta-galactosyl-containing glycoconjugates on the cell  surface and in the extracellular matrix (Cerra  et al., 1984;  Merkle and Cummings, 1988;	bind
15931	3	5540	7	10	NULL	NULL	NULL	statement 2	Process		is inactive					reducing agents	Chemical	in the absence of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_10_5198_s_18	7890630	(i) Galectin-1 is found  mainly in the cytosol of most cells in which it occurs (Briles  et  al., 1979), (ii) the lectin has free sulfhydryls and is inactive  in the absence of reducing agents (Hirabayashi and Kasai, 1991;  Barondes, 1984), (iii) the lectin lacks an identifiable signal sequence  and does not appear to be secreted through the normal secretory pathway  in differentiated myoblasts (Cooper and Barondes, 1990), (iv) the  lectin binds to beta-galactosyl-containing glycoconjugates on the cell  surface and in the extracellular matrix (Cerra  et al., 1984;  Merkle and Cummings, 1988;	bind
15933	4	5540	7	10	NULL	NULL	NULL	Lectin	GP		lacks					Signal sequence	GP	 an identifiable			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_10_5198_s_18	7890630	(i) Galectin-1 is found  mainly in the cytosol of most cells in which it occurs (Briles  et  al., 1979), (ii) the lectin has free sulfhydryls and is inactive  in the absence of reducing agents (Hirabayashi and Kasai, 1991;  Barondes, 1984), (iii) the lectin lacks an identifiable signal sequence  and does not appear to be secreted through the normal secretory pathway  in differentiated myoblasts (Cooper and Barondes, 1990), (iv) the  lectin binds to beta-galactosyl-containing glycoconjugates on the cell  surface and in the extracellular matrix (Cerra  et al., 1984;  Merkle and Cummings, 1988;	bind
15934	5	5540	7	10	NULL	NULL	NULL	Lectin	GP		is not secreted through					secretory pathway	Process	normal 			NULL	differentiated myoblasts 	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_10_5198_s_18	7890630	(i) Galectin-1 is found  mainly in the cytosol of most cells in which it occurs (Briles  et  al., 1979), (ii) the lectin has free sulfhydryls and is inactive  in the absence of reducing agents (Hirabayashi and Kasai, 1991;  Barondes, 1984), (iii) the lectin lacks an identifiable signal sequence  and does not appear to be secreted through the normal secretory pathway  in differentiated myoblasts (Cooper and Barondes, 1990), (iv) the  lectin binds to beta-galactosyl-containing glycoconjugates on the cell  surface and in the extracellular matrix (Cerra  et al., 1984;  Merkle and Cummings, 1988;	bind
15936	7	5540	7	10	NULL	NULL	NULL	beta-galactosyl-containing glycoconjugates	Chemical		bind					lectin	GP				NULL	 cell surface	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_10_5198_s_18	7890630	(i) Galectin-1 is found  mainly in the cytosol of most cells in which it occurs (Briles  et  al., 1979), (ii) the lectin has free sulfhydryls and is inactive  in the absence of reducing agents (Hirabayashi and Kasai, 1991;  Barondes, 1984), (iii) the lectin lacks an identifiable signal sequence  and does not appear to be secreted through the normal secretory pathway  in differentiated myoblasts (Cooper and Barondes, 1990), (iv) the  lectin binds to beta-galactosyl-containing glycoconjugates on the cell  surface and in the extracellular matrix (Cerra  et al., 1984;  Merkle and Cummings, 1988;	bind
15937	8	5540	7	10	NULL	NULL	NULL	beta-galactosyl-containing glycoconjugates	Chemical		binds					lectin	GP				NULL	extracellular matrix 	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_10_5198_s_18	7890630	(i) Galectin-1 is found  mainly in the cytosol of most cells in which it occurs (Briles  et  al., 1979), (ii) the lectin has free sulfhydryls and is inactive  in the absence of reducing agents (Hirabayashi and Kasai, 1991;  Barondes, 1984), (iii) the lectin lacks an identifiable signal sequence  and does not appear to be secreted through the normal secretory pathway  in differentiated myoblasts (Cooper and Barondes, 1990), (iv) the  lectin binds to beta-galactosyl-containing glycoconjugates on the cell  surface and in the extracellular matrix (Cerra  et al., 1984;  Merkle and Cummings, 1988;	bind
16572	1	5541	6	10	NULL	NULL	NULL	GDP	Chemical		bind					Arf-1	GP	membrane attached			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_7_1199_s_239	11748249	(I) GDP bound to Arf-1 attached to the membrane is replaced with GTP by Arf-1 guanine exchange factor.	bind
16573	2	5541	6	10	NULL	NULL	NULL	GTP	Chemical		bind					Arf-1	GP	membrane attached			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_7_1199_s_239	11748249	(I) GDP bound to Arf-1 attached to the membrane is replaced with GTP by Arf-1 guanine exchange factor.	bind
16574	3	5541	6	10	NULL	NULL	NULL	statement 1	Process		is replaced by					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_7_1199_s_239	11748249	(I) GDP bound to Arf-1 attached to the membrane is replaced with GTP by Arf-1 guanine exchange factor.	bind
44827	4	5541	6	10	NULL	NULL	NULL	statement 2	Process		occurs through					Arf-1 guanine exchange factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_7_1199_s_239	11748249	(I) GDP bound to Arf-1 attached to the membrane is replaced with GTP by Arf-1 guanine exchange factor.	bind
15940	1	5541	7	10	NULL	NULL	NULL	GDP	Chemical		bind					Arf-1	GP	membrane attached			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_7_1199_s_239	11748249	(I) GDP bound to Arf-1 attached to the membrane is replaced with GTP by Arf-1 guanine exchange factor.	bind
15941	2	5541	7	NULL	NULL	0	NULL	GTP	NULL		binds	NULL				 Arf-1	NULL	membrane attached			NULL		0	NULL	NULL	NULL	gw60_cellbiol_155_7_1199_s_239	11748249	(I) GDP bound to Arf-1 attached to the membrane is replaced with GTP by Arf-1 guanine exchange factor.	bind
15942	3	5541	7	10	NULL	NULL	NULL	statement 1	Process		is replaced by					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_7_1199_s_239	11748249	(I) GDP bound to Arf-1 attached to the membrane is replaced with GTP by Arf-1 guanine exchange factor.	bind
15943	4	5541	7	10	NULL	NULL	NULL	statement 2	Process		occurs through					Arf-1 guanine exchange factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_7_1199_s_239	11748249	(I) GDP bound to Arf-1 attached to the membrane is replaced with GTP by Arf-1 guanine exchange factor.	bind
16722	1	5542	6	10	NULL	NULL	NULL	GTP	Chemical		bind					eRF3	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45693_s_269	15337765	(i) GTP-bound eRF3 associates with eRF1 and brings it to the ribosomal A site, (ii) the association of eRF3 with the GTPase-activating proteins consisting of ribosome and eRF1 leads to the activation of GTP hydrolysis, and (iii) the resulting GDP-bound form of eRF3 dissociates from eRF1, although its lifetime may be quite short in the presence of Mg2+.	bind
16723	2	5542	6	10	NULL	NULL	NULL	statement 1	Process		associates with					eRF1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45693_s_269	15337765	(i) GTP-bound eRF3 associates with eRF1 and brings it to the ribosomal A site, (ii) the association of eRF3 with the GTPase-activating proteins consisting of ribosome and eRF1 leads to the activation of GTP hydrolysis, and (iii) the resulting GDP-bound form of eRF3 dissociates from eRF1, although its lifetime may be quite short in the presence of Mg2+.	bind
16724	3	5542	6	10	NULL	NULL	NULL	eRF1	GP		enters to					ribosome	CellComponent		 A site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45693_s_269	15337765	(i) GTP-bound eRF3 associates with eRF1 and brings it to the ribosomal A site, (ii) the association of eRF3 with the GTPase-activating proteins consisting of ribosome and eRF1 leads to the activation of GTP hydrolysis, and (iii) the resulting GDP-bound form of eRF3 dissociates from eRF1, although its lifetime may be quite short in the presence of Mg2+.	bind
16725	4	5542	6	10	NULL	NULL	NULL	statement 2	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45693_s_269	15337765	(i) GTP-bound eRF3 associates with eRF1 and brings it to the ribosomal A site, (ii) the association of eRF3 with the GTPase-activating proteins consisting of ribosome and eRF1 leads to the activation of GTP hydrolysis, and (iii) the resulting GDP-bound form of eRF3 dissociates from eRF1, although its lifetime may be quite short in the presence of Mg2+.	bind
16727	5	5542	6	10	NULL	NULL	NULL	GTPase-activating proteins	GP		consists of					ribosome	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45693_s_269	15337765	(i) GTP-bound eRF3 associates with eRF1 and brings it to the ribosomal A site, (ii) the association of eRF3 with the GTPase-activating proteins consisting of ribosome and eRF1 leads to the activation of GTP hydrolysis, and (iii) the resulting GDP-bound form of eRF3 dissociates from eRF1, although its lifetime may be quite short in the presence of Mg2+.	bind
16728	6	5542	6	10	NULL	NULL	NULL	eRF3	GP		associates with					statement 11	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45693_s_269	15337765	(i) GTP-bound eRF3 associates with eRF1 and brings it to the ribosomal A site, (ii) the association of eRF3 with the GTPase-activating proteins consisting of ribosome and eRF1 leads to the activation of GTP hydrolysis, and (iii) the resulting GDP-bound form of eRF3 dissociates from eRF1, although its lifetime may be quite short in the presence of Mg2+.	bind
16731	7	5542	6	10	NULL	NULL	NULL	statement 6	Process		activates					GTP	Chemical	hydrolysis of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45693_s_269	15337765	(i) GTP-bound eRF3 associates with eRF1 and brings it to the ribosomal A site, (ii) the association of eRF3 with the GTPase-activating proteins consisting of ribosome and eRF1 leads to the activation of GTP hydrolysis, and (iii) the resulting GDP-bound form of eRF3 dissociates from eRF1, although its lifetime may be quite short in the presence of Mg2+.	bind
16732	8	5542	6	10	NULL	NULL	NULL	GDP	Chemical		bind					eRF3	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45693_s_269	15337765	(i) GTP-bound eRF3 associates with eRF1 and brings it to the ribosomal A site, (ii) the association of eRF3 with the GTPase-activating proteins consisting of ribosome and eRF1 leads to the activation of GTP hydrolysis, and (iii) the resulting GDP-bound form of eRF3 dissociates from eRF1, although its lifetime may be quite short in the presence of Mg2+.	bind
16733	9	5542	6	10	NULL	NULL	NULL	statement 8	Process		dissociates from					eRF1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45693_s_269	15337765	(i) GTP-bound eRF3 associates with eRF1 and brings it to the ribosomal A site, (ii) the association of eRF3 with the GTPase-activating proteins consisting of ribosome and eRF1 leads to the activation of GTP hydrolysis, and (iii) the resulting GDP-bound form of eRF3 dissociates from eRF1, although its lifetime may be quite short in the presence of Mg2+.	bind
53107	10	5542	6	10	NULL	NULL	NULL	GTPase-activating proteins	GP		consists of					eRF1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45693_s_269	15337765	(i) GTP-bound eRF3 associates with eRF1 and brings it to the ribosomal A site, (ii) the association of eRF3 with the GTPase-activating proteins consisting of ribosome and eRF1 leads to the activation of GTP hydrolysis, and (iii) the resulting GDP-bound form of eRF3 dissociates from eRF1, although its lifetime may be quite short in the presence of Mg2+.	bind
53108	11	5542	6	10	NULL	NULL	NULL	statement 5	Process		occurs along with					statement 10	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45693_s_269	15337765	(i) GTP-bound eRF3 associates with eRF1 and brings it to the ribosomal A site, (ii) the association of eRF3 with the GTPase-activating proteins consisting of ribosome and eRF1 leads to the activation of GTP hydrolysis, and (iii) the resulting GDP-bound form of eRF3 dissociates from eRF1, although its lifetime may be quite short in the presence of Mg2+.	bind
15944	1	5542	7	10	NULL	NULL	NULL	GTP	Chemical		bind					 eRF3	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45693_s_269	15337765	(i) GTP-bound eRF3 associates with eRF1 and brings it to the ribosomal A site, (ii) the association of eRF3 with the GTPase-activating proteins consisting of ribosome and eRF1 leads to the activation of GTP hydrolysis, and (iii) the resulting GDP-bound form of eRF3 dissociates from eRF1, although its lifetime may be quite short in the presence of Mg2+.	bind
15945	3	5542	7	10	NULL	NULL	NULL	eRF1	GP		enters					ribosome	CellComponent		A site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45693_s_269	15337765	(i) GTP-bound eRF3 associates with eRF1 and brings it to the ribosomal A site, (ii) the association of eRF3 with the GTPase-activating proteins consisting of ribosome and eRF1 leads to the activation of GTP hydrolysis, and (iii) the resulting GDP-bound form of eRF3 dissociates from eRF1, although its lifetime may be quite short in the presence of Mg2+.	bind
15946	4	5542	7	10	NULL	NULL	NULL	GTPase-activating protein	GP		consist of					ribosome	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45693_s_269	15337765	(i) GTP-bound eRF3 associates with eRF1 and brings it to the ribosomal A site, (ii) the association of eRF3 with the GTPase-activating proteins consisting of ribosome and eRF1 leads to the activation of GTP hydrolysis, and (iii) the resulting GDP-bound form of eRF3 dissociates from eRF1, although its lifetime may be quite short in the presence of Mg2+.	bind
15947	5	5542	7	10	NULL	NULL	NULL	GTPase-activating protein	GP		consist of					eRF1 	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45693_s_269	15337765	(i) GTP-bound eRF3 associates with eRF1 and brings it to the ribosomal A site, (ii) the association of eRF3 with the GTPase-activating proteins consisting of ribosome and eRF1 leads to the activation of GTP hydrolysis, and (iii) the resulting GDP-bound form of eRF3 dissociates from eRF1, although its lifetime may be quite short in the presence of Mg2+.	bind
15948	6	5542	7	10	NULL	NULL	NULL	statement 3	Process		occurs along with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45693_s_269	15337765	(i) GTP-bound eRF3 associates with eRF1 and brings it to the ribosomal A site, (ii) the association of eRF3 with the GTPase-activating proteins consisting of ribosome and eRF1 leads to the activation of GTP hydrolysis, and (iii) the resulting GDP-bound form of eRF3 dissociates from eRF1, although its lifetime may be quite short in the presence of Mg2+.	bind
15949	7	5542	7	10	NULL	NULL	NULL	eRF3	GP		associate with					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45693_s_269	15337765	(i) GTP-bound eRF3 associates with eRF1 and brings it to the ribosomal A site, (ii) the association of eRF3 with the GTPase-activating proteins consisting of ribosome and eRF1 leads to the activation of GTP hydrolysis, and (iii) the resulting GDP-bound form of eRF3 dissociates from eRF1, although its lifetime may be quite short in the presence of Mg2+.	bind
15950	8	5542	7	10	NULL	NULL	NULL	statement 7	Process		activates					GTP	Chemical	hydrolysis of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45693_s_269	15337765	(i) GTP-bound eRF3 associates with eRF1 and brings it to the ribosomal A site, (ii) the association of eRF3 with the GTPase-activating proteins consisting of ribosome and eRF1 leads to the activation of GTP hydrolysis, and (iii) the resulting GDP-bound form of eRF3 dissociates from eRF1, although its lifetime may be quite short in the presence of Mg2+.	bind
15951	10	5542	7	10	NULL	NULL	NULL	statement 9	Process		dissociates from					eRF1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45693_s_269	15337765	(i) GTP-bound eRF3 associates with eRF1 and brings it to the ribosomal A site, (ii) the association of eRF3 with the GTPase-activating proteins consisting of ribosome and eRF1 leads to the activation of GTP hydrolysis, and (iii) the resulting GDP-bound form of eRF3 dissociates from eRF1, although its lifetime may be quite short in the presence of Mg2+.	bind
44848	2	5542	7	10	NULL	NULL	NULL	statement 1	Process		associate with					eRF1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45693_s_269	15337765	(i) GTP-bound eRF3 associates with eRF1 and brings it to the ribosomal A site, (ii) the association of eRF3 with the GTPase-activating proteins consisting of ribosome and eRF1 leads to the activation of GTP hydrolysis, and (iii) the resulting GDP-bound form of eRF3 dissociates from eRF1, although its lifetime may be quite short in the presence of Mg2+.	bind
44849	9	5542	7	10	NULL	NULL	NULL	GDP	Chemical		bind					eRF3	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45693_s_269	15337765	(i) GTP-bound eRF3 associates with eRF1 and brings it to the ribosomal A site, (ii) the association of eRF3 with the GTPase-activating proteins consisting of ribosome and eRF1 leads to the activation of GTP hydrolysis, and (iii) the resulting GDP-bound form of eRF3 dissociates from eRF1, although its lifetime may be quite short in the presence of Mg2+.	bind
53106	11	5542	7	10	NULL	NULL	NULL	statement 2			leads to					statement 3					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45693_s_269	15337765	(i) GTP-bound eRF3 associates with eRF1 and brings it to the ribosomal A site, (ii) the association of eRF3 with the GTPase-activating proteins consisting of ribosome and eRF1 leads to the activation of GTP hydrolysis, and (iii) the resulting GDP-bound form of eRF3 dissociates from eRF1, although its lifetime may be quite short in the presence of Mg2+.	bind
16718	1	5543	6	10	NULL	NULL	NULL	t-RNA	NucleicAcid		bind					A-site	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_19_5241_s_227	11013226	(i) His229 might be involved in the binding of adenosine 76 of the A-site-bound tRNA.	bind
16719	2	5543	6	10	NULL	NULL	NULL				be involved in		might	His229		statement 1	Process	binding of	adenosine 76		NULL		NULL	NULL	NULL	NULL	gw60_embo_19_19_5241_s_227	11013226	(i) His229 might be involved in the binding of adenosine 76 of the A-site-bound tRNA.	bind
15953	2	5543	7	10	NULL	NULL	NULL				be involved in		might	His229		statement 1	Process		adenosine 76 		NULL		NULL	NULL	NULL	NULL	gw60_embo_19_19_5241_s_227	11013226	(i) His229 might be involved in the binding of adenosine 76 of the A-site-bound tRNA.	bind
19758	1	5543	7	10	NULL	NULL	NULL	tRNA	NucleicAcid		bind					A site	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_19_5241_s_227	11013226	(i) His229 might be involved in the binding of adenosine 76 of the A-site-bound tRNA.	bind
16598	1	5544	6	10	NULL	NULL	NULL	HSP-CBF	GP		bind					NF-Y	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_28_26332_s_237	11306579	(i) HSP-CBF might intervene early during the establishment of an open chromatin configuration within the heat shock regulatory regions following NF-Y binding (Fig.  7 A).	bind
16599	2	5544	6	10	NULL	NULL	NULL	statement 1	Process		intervene during		might			open chromatin configuration	Process	establishement of		heat shock regulatory region	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_28_26332_s_237	11306579	(i) HSP-CBF might intervene early during the establishment of an open chromatin configuration within the heat shock regulatory regions following NF-Y binding (Fig.  7 A).	bind
44810	3	5544	6	10	NULL	NULL	NULL	statement 2	Process		occurs following					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_28_26332_s_237	11306579	(i) HSP-CBF might intervene early during the establishment of an open chromatin configuration within the heat shock regulatory regions following NF-Y binding (Fig.  7 A).	bind
15954	1	5544	7	10	NULL	NULL	NULL	HSP-CBF	GP		intervene during		might;;early			open chromatin configuration	Process	establishment of		heat shock regulatory regions	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_28_26332_s_237	11306579	(i) HSP-CBF might intervene early during the establishment of an open chromatin configuration within the heat shock regulatory regions following NF-Y binding (Fig.  7 A).	bind
15956	2	5544	7	10	NULL	NULL	NULL	statement 1	Process		occurs upon					NF-Y	GP	binding of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_28_26332_s_237	11306579	(i) HSP-CBF might intervene early during the establishment of an open chromatin configuration within the heat shock regulatory regions following NF-Y binding (Fig.  7 A).	bind
16601	1	5545	6	10	NULL	NULL	NULL	bd receptor	GP		is a type of					K88 adhesin receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_1_165_s_283	9864211	(i) In addition to being found in phenotype D animals, receptor  d (IGLad) is also found in phenotype A animals, and (ii) receptor  d is not present in phenotype C animals, indicating that there may be a fourth K88 adhesin receptor, possibly a  bd receptor that binds both K88ab and K88ad adhesin and is found exclusively in phenotype C animals.	bind
16602	2	5545	6	10	NULL	NULL	NULL	bd receptor	GP		bind					adhesin	GP		K88ab		NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_1_165_s_283	9864211	(i) In addition to being found in phenotype D animals, receptor  d (IGLad) is also found in phenotype A animals, and (ii) receptor  d is not present in phenotype C animals, indicating that there may be a fourth K88 adhesin receptor, possibly a  bd receptor that binds both K88ab and K88ad adhesin and is found exclusively in phenotype C animals.	bind
16603	3	5545	6	10	NULL	NULL	NULL	bd receptor	GP		bind					adhesin	GP		K88ad		NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_1_165_s_283	9864211	(i) In addition to being found in phenotype D animals, receptor  d (IGLad) is also found in phenotype A animals, and (ii) receptor  d is not present in phenotype C animals, indicating that there may be a fourth K88 adhesin receptor, possibly a  bd receptor that binds both K88ab and K88ad adhesin and is found exclusively in phenotype C animals.	bind
16606	4	5545	6	10	NULL	NULL	NULL	bd receptor	GP		is found		exclusively			phenotype C animals	Organism				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_1_165_s_283	9864211	(i) In addition to being found in phenotype D animals, receptor  d (IGLad) is also found in phenotype A animals, and (ii) receptor  d is not present in phenotype C animals, indicating that there may be a fourth K88 adhesin receptor, possibly a  bd receptor that binds both K88ab and K88ad adhesin and is found exclusively in phenotype C animals.	bind
16607	5	5545	6	10	NULL	NULL	NULL	receptor d	GP		is					IGLad	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_1_165_s_283	9864211	(i) In addition to being found in phenotype D animals, receptor  d (IGLad) is also found in phenotype A animals, and (ii) receptor  d is not present in phenotype C animals, indicating that there may be a fourth K88 adhesin receptor, possibly a  bd receptor that binds both K88ab and K88ad adhesin and is found exclusively in phenotype C animals.	bind
16608	6	5545	6	10	NULL	NULL	NULL	receptor d	GP		is found in					phenotype A animals	Organism				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_1_165_s_283	9864211	(i) In addition to being found in phenotype D animals, receptor  d (IGLad) is also found in phenotype A animals, and (ii) receptor  d is not present in phenotype C animals, indicating that there may be a fourth K88 adhesin receptor, possibly a  bd receptor that binds both K88ab and K88ad adhesin and is found exclusively in phenotype C animals.	bind
16609	7	5545	6	10	NULL	NULL	NULL	receptor d	GP		is not present in					phenotype C animals	Organism				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_1_165_s_283	9864211	(i) In addition to being found in phenotype D animals, receptor  d (IGLad) is also found in phenotype A animals, and (ii) receptor  d is not present in phenotype C animals, indicating that there may be a fourth K88 adhesin receptor, possibly a  bd receptor that binds both K88ab and K88ad adhesin and is found exclusively in phenotype C animals.	bind
15957	2	5545	7	10	NULL	NULL	NULL	bd receptor	GP		bind					adhesin 	GP		K88ab		NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_1_165_s_283	9864211	(i) In addition to being found in phenotype D animals, receptor  d (IGLad) is also found in phenotype A animals, and (ii) receptor  d is not present in phenotype C animals, indicating that there may be a fourth K88 adhesin receptor, possibly a  bd receptor that binds both K88ab and K88ad adhesin and is found exclusively in phenotype C animals.	bind
15958	3	5545	7	10	NULL	NULL	NULL	bd receptor	GP		bind					adhesin	GP		K88ad		NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_1_165_s_283	9864211	(i) In addition to being found in phenotype D animals, receptor  d (IGLad) is also found in phenotype A animals, and (ii) receptor  d is not present in phenotype C animals, indicating that there may be a fourth K88 adhesin receptor, possibly a  bd receptor that binds both K88ab and K88ad adhesin and is found exclusively in phenotype C animals.	bind
44926	1	5545	7	10	NULL	NULL	NULL	bd receptor	GP		is a type of					K88 adhesin receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_1_165_s_283	9864211	(i) In addition to being found in phenotype D animals, receptor  d (IGLad) is also found in phenotype A animals, and (ii) receptor  d is not present in phenotype C animals, indicating that there may be a fourth K88 adhesin receptor, possibly a  bd receptor that binds both K88ab and K88ad adhesin and is found exclusively in phenotype C animals.	bind
44927	5	5545	7	10	NULL	NULL	NULL	receptor d	GP		is 					IGLad	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_1_165_s_283	9864211	(i) In addition to being found in phenotype D animals, receptor  d (IGLad) is also found in phenotype A animals, and (ii) receptor  d is not present in phenotype C animals, indicating that there may be a fourth K88 adhesin receptor, possibly a  bd receptor that binds both K88ab and K88ad adhesin and is found exclusively in phenotype C animals.	bind
44928	4	5545	7	10	NULL	NULL	NULL	bd receptor	GP		found in		exclusively			phenotype C animals	Organism				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_1_165_s_283	9864211	(i) In addition to being found in phenotype D animals, receptor  d (IGLad) is also found in phenotype A animals, and (ii) receptor  d is not present in phenotype C animals, indicating that there may be a fourth K88 adhesin receptor, possibly a  bd receptor that binds both K88ab and K88ad adhesin and is found exclusively in phenotype C animals.	bind
44929	6	5545	7	10	NULL	NULL	NULL	receptor d	GP		is found in					phenotype D animals	Organism				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_1_165_s_283	9864211	(i) In addition to being found in phenotype D animals, receptor  d (IGLad) is also found in phenotype A animals, and (ii) receptor  d is not present in phenotype C animals, indicating that there may be a fourth K88 adhesin receptor, possibly a  bd receptor that binds both K88ab and K88ad adhesin and is found exclusively in phenotype C animals.	bind
44930	7	5545	7	10	NULL	NULL	NULL	receptor d	GP		is found in					phenotype A animals	Organism				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_1_165_s_283	9864211	(i) In addition to being found in phenotype D animals, receptor  d (IGLad) is also found in phenotype A animals, and (ii) receptor  d is not present in phenotype C animals, indicating that there may be a fourth K88 adhesin receptor, possibly a  bd receptor that binds both K88ab and K88ad adhesin and is found exclusively in phenotype C animals.	bind
44931	8	5545	7	10	NULL	NULL	NULL	receptor d	GP		is not found in					phenotype C animals	Organism				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_1_165_s_283	9864211	(i) In addition to being found in phenotype D animals, receptor  d (IGLad) is also found in phenotype A animals, and (ii) receptor  d is not present in phenotype C animals, indicating that there may be a fourth K88 adhesin receptor, possibly a  bd receptor that binds both K88ab and K88ad adhesin and is found exclusively in phenotype C animals.	bind
16708	1	5546	6	10	NULL	NULL	NULL	A. naeslundii genospecies 2	Organism	human	bind		avidly			PRPs	GP	acidic			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7224_s_108	11705891	(i) In preferential acidic-PRP binding, oral strains of  A. naeslundii genospecies 2 of human ( n = 11) and monkey ( n = 2) origin bound avidly to acidic PRPs but deviated in their relative, although weak, capacities for binding to statherin and oral strains of  A. naeslundii genospecies 1 bound either avidly ( n = 2) or weakly ( n = 4) to acidic PRPs. (ii) In preferential statherin binding,  A. viscosus strains from rat or hamster plaque ( n = 6) and a case of human actinomycosis bound statherin avidly and preferentially.	bind
16709	2	5546	6	10	NULL	NULL	NULL	A. naeslundii genospecies 2	Organism	monkey	bind		avidly			PRPs	GP	acidic			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7224_s_108	11705891	(i) In preferential acidic-PRP binding, oral strains of  A. naeslundii genospecies 2 of human ( n = 11) and monkey ( n = 2) origin bound avidly to acidic PRPs but deviated in their relative, although weak, capacities for binding to statherin and oral strains of  A. naeslundii genospecies 1 bound either avidly ( n = 2) or weakly ( n = 4) to acidic PRPs. (ii) In preferential statherin binding,  A. viscosus strains from rat or hamster plaque ( n = 6) and a case of human actinomycosis bound statherin avidly and preferentially.	bind
16710	3	5546	6	10	NULL	NULL	NULL	A. naeslundii genospecies 2	Organism	human	bind		weakly			statherin	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7224_s_108	11705891	(i) In preferential acidic-PRP binding, oral strains of  A. naeslundii genospecies 2 of human ( n = 11) and monkey ( n = 2) origin bound avidly to acidic PRPs but deviated in their relative, although weak, capacities for binding to statherin and oral strains of  A. naeslundii genospecies 1 bound either avidly ( n = 2) or weakly ( n = 4) to acidic PRPs. (ii) In preferential statherin binding,  A. viscosus strains from rat or hamster plaque ( n = 6) and a case of human actinomycosis bound statherin avidly and preferentially.	bind
16711	4	5546	6	10	NULL	NULL	NULL	A. naeslundii genospecies 2	Organism	monkey	bind		weakly			statherin	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7224_s_108	11705891	(i) In preferential acidic-PRP binding, oral strains of  A. naeslundii genospecies 2 of human ( n = 11) and monkey ( n = 2) origin bound avidly to acidic PRPs but deviated in their relative, although weak, capacities for binding to statherin and oral strains of  A. naeslundii genospecies 1 bound either avidly ( n = 2) or weakly ( n = 4) to acidic PRPs. (ii) In preferential statherin binding,  A. viscosus strains from rat or hamster plaque ( n = 6) and a case of human actinomycosis bound statherin avidly and preferentially.	bind
16712	5	5546	6	10	NULL	NULL	NULL	A. naeslundii genospecies 1	Organism		bind		avidly			PRPs	GP	acidic			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7224_s_108	11705891	(i) In preferential acidic-PRP binding, oral strains of  A. naeslundii genospecies 2 of human ( n = 11) and monkey ( n = 2) origin bound avidly to acidic PRPs but deviated in their relative, although weak, capacities for binding to statherin and oral strains of  A. naeslundii genospecies 1 bound either avidly ( n = 2) or weakly ( n = 4) to acidic PRPs. (ii) In preferential statherin binding,  A. viscosus strains from rat or hamster plaque ( n = 6) and a case of human actinomycosis bound statherin avidly and preferentially.	bind
16713	6	5546	6	10	NULL	NULL	NULL	A. naeslundii genospecies 1	Organism		bind		weakly			PRP	GP	acidic			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7224_s_108	11705891	(i) In preferential acidic-PRP binding, oral strains of  A. naeslundii genospecies 2 of human ( n = 11) and monkey ( n = 2) origin bound avidly to acidic PRPs but deviated in their relative, although weak, capacities for binding to statherin and oral strains of  A. naeslundii genospecies 1 bound either avidly ( n = 2) or weakly ( n = 4) to acidic PRPs. (ii) In preferential statherin binding,  A. viscosus strains from rat or hamster plaque ( n = 6) and a case of human actinomycosis bound statherin avidly and preferentially.	bind
16714	7	5546	6	10	NULL	NULL	NULL	statement 5	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7224_s_108	11705891	(i) In preferential acidic-PRP binding, oral strains of  A. naeslundii genospecies 2 of human ( n = 11) and monkey ( n = 2) origin bound avidly to acidic PRPs but deviated in their relative, although weak, capacities for binding to statherin and oral strains of  A. naeslundii genospecies 1 bound either avidly ( n = 2) or weakly ( n = 4) to acidic PRPs. (ii) In preferential statherin binding,  A. viscosus strains from rat or hamster plaque ( n = 6) and a case of human actinomycosis bound statherin avidly and preferentially.	bind
16715	8	5546	6	10	NULL	NULL	NULL	A. viscosus strains	Organism	rat	bind		avidly;;preferentially			statherin	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7224_s_108	11705891	(i) In preferential acidic-PRP binding, oral strains of  A. naeslundii genospecies 2 of human ( n = 11) and monkey ( n = 2) origin bound avidly to acidic PRPs but deviated in their relative, although weak, capacities for binding to statherin and oral strains of  A. naeslundii genospecies 1 bound either avidly ( n = 2) or weakly ( n = 4) to acidic PRPs. (ii) In preferential statherin binding,  A. viscosus strains from rat or hamster plaque ( n = 6) and a case of human actinomycosis bound statherin avidly and preferentially.	bind
16716	9	5546	6	10	NULL	NULL	NULL	A. viscosus strains	Organism	hamster	bind		avidly;;preferentially			statherin	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7224_s_108	11705891	(i) In preferential acidic-PRP binding, oral strains of  A. naeslundii genospecies 2 of human ( n = 11) and monkey ( n = 2) origin bound avidly to acidic PRPs but deviated in their relative, although weak, capacities for binding to statherin and oral strains of  A. naeslundii genospecies 1 bound either avidly ( n = 2) or weakly ( n = 4) to acidic PRPs. (ii) In preferential statherin binding,  A. viscosus strains from rat or hamster plaque ( n = 6) and a case of human actinomycosis bound statherin avidly and preferentially.	bind
16717	10	5546	6	10	NULL	NULL	NULL	actinomycosis	Organism	human	bind		avidly;;preferentially			statherin	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7224_s_108	11705891	(i) In preferential acidic-PRP binding, oral strains of  A. naeslundii genospecies 2 of human ( n = 11) and monkey ( n = 2) origin bound avidly to acidic PRPs but deviated in their relative, although weak, capacities for binding to statherin and oral strains of  A. naeslundii genospecies 1 bound either avidly ( n = 2) or weakly ( n = 4) to acidic PRPs. (ii) In preferential statherin binding,  A. viscosus strains from rat or hamster plaque ( n = 6) and a case of human actinomycosis bound statherin avidly and preferentially.	bind
15959	1	5546	7	10	NULL	NULL	NULL	 A. naeslundii	Organism	genospecies 2 of human origin	bind		avidly			PRPs	GP	acidic			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7224_s_108	11705891	(i) In preferential acidic-PRP binding, oral strains of  A. naeslundii genospecies 2 of human ( n = 11) and monkey ( n = 2) origin bound avidly to acidic PRPs but deviated in their relative, although weak, capacities for binding to statherin and oral strains of  A. naeslundii genospecies 1 bound either avidly ( n = 2) or weakly ( n = 4) to acidic PRPs. (ii) In preferential statherin binding,  A. viscosus strains from rat or hamster plaque ( n = 6) and a case of human actinomycosis bound statherin avidly and preferentially.	bind
15960	2	5546	7	10	NULL	NULL	NULL	A. naeslundii	Organism	genospecies 2 of monkey origin	bind		avidly			PRPs	GP	acidic			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7224_s_108	11705891	(i) In preferential acidic-PRP binding, oral strains of  A. naeslundii genospecies 2 of human ( n = 11) and monkey ( n = 2) origin bound avidly to acidic PRPs but deviated in their relative, although weak, capacities for binding to statherin and oral strains of  A. naeslundii genospecies 1 bound either avidly ( n = 2) or weakly ( n = 4) to acidic PRPs. (ii) In preferential statherin binding,  A. viscosus strains from rat or hamster plaque ( n = 6) and a case of human actinomycosis bound statherin avidly and preferentially.	bind
15961	3	5546	7	10	NULL	NULL	NULL	A. naeslundii 	Organism	genospecies 2 of human origin	bind		weakly			statherin	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7224_s_108	11705891	(i) In preferential acidic-PRP binding, oral strains of  A. naeslundii genospecies 2 of human ( n = 11) and monkey ( n = 2) origin bound avidly to acidic PRPs but deviated in their relative, although weak, capacities for binding to statherin and oral strains of  A. naeslundii genospecies 1 bound either avidly ( n = 2) or weakly ( n = 4) to acidic PRPs. (ii) In preferential statherin binding,  A. viscosus strains from rat or hamster plaque ( n = 6) and a case of human actinomycosis bound statherin avidly and preferentially.	bind
15962	4	5546	7	10	NULL	NULL	NULL	A. naeslundii	Organism	genospecies 2 of monkey origin	bind		weakly			statherin	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7224_s_108	11705891	(i) In preferential acidic-PRP binding, oral strains of  A. naeslundii genospecies 2 of human ( n = 11) and monkey ( n = 2) origin bound avidly to acidic PRPs but deviated in their relative, although weak, capacities for binding to statherin and oral strains of  A. naeslundii genospecies 1 bound either avidly ( n = 2) or weakly ( n = 4) to acidic PRPs. (ii) In preferential statherin binding,  A. viscosus strains from rat or hamster plaque ( n = 6) and a case of human actinomycosis bound statherin avidly and preferentially.	bind
15963	5	5546	7	10	NULL	NULL	NULL	A. naeslundii	Organism	genospecies 1	bind		avidly			PRPs	GP	acidic			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7224_s_108	11705891	(i) In preferential acidic-PRP binding, oral strains of  A. naeslundii genospecies 2 of human ( n = 11) and monkey ( n = 2) origin bound avidly to acidic PRPs but deviated in their relative, although weak, capacities for binding to statherin and oral strains of  A. naeslundii genospecies 1 bound either avidly ( n = 2) or weakly ( n = 4) to acidic PRPs. (ii) In preferential statherin binding,  A. viscosus strains from rat or hamster plaque ( n = 6) and a case of human actinomycosis bound statherin avidly and preferentially.	bind
15964	6	5546	7	10	NULL	NULL	NULL	A. naeslundii	Organism	genospecies 1	bind		weakly			PRPs	GP	acidic			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7224_s_108	11705891	(i) In preferential acidic-PRP binding, oral strains of  A. naeslundii genospecies 2 of human ( n = 11) and monkey ( n = 2) origin bound avidly to acidic PRPs but deviated in their relative, although weak, capacities for binding to statherin and oral strains of  A. naeslundii genospecies 1 bound either avidly ( n = 2) or weakly ( n = 4) to acidic PRPs. (ii) In preferential statherin binding,  A. viscosus strains from rat or hamster plaque ( n = 6) and a case of human actinomycosis bound statherin avidly and preferentially.	bind
15965	7	5546	7	10	NULL	NULL	NULL	statement 5	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7224_s_108	11705891	(i) In preferential acidic-PRP binding, oral strains of  A. naeslundii genospecies 2 of human ( n = 11) and monkey ( n = 2) origin bound avidly to acidic PRPs but deviated in their relative, although weak, capacities for binding to statherin and oral strains of  A. naeslundii genospecies 1 bound either avidly ( n = 2) or weakly ( n = 4) to acidic PRPs. (ii) In preferential statherin binding,  A. viscosus strains from rat or hamster plaque ( n = 6) and a case of human actinomycosis bound statherin avidly and preferentially.	bind
15966	8	5546	7	10	NULL	NULL	NULL	A. viscosus	Organism	rat	bind		avidly;;preferentially			statherin 	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7224_s_108	11705891	(i) In preferential acidic-PRP binding, oral strains of  A. naeslundii genospecies 2 of human ( n = 11) and monkey ( n = 2) origin bound avidly to acidic PRPs but deviated in their relative, although weak, capacities for binding to statherin and oral strains of  A. naeslundii genospecies 1 bound either avidly ( n = 2) or weakly ( n = 4) to acidic PRPs. (ii) In preferential statherin binding,  A. viscosus strains from rat or hamster plaque ( n = 6) and a case of human actinomycosis bound statherin avidly and preferentially.	bind
15967	9	5546	7	10	NULL	NULL	NULL	A. viscosus	Organism	hamster plaque	bind		avidly;;preferentially			statherin	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7224_s_108	11705891	(i) In preferential acidic-PRP binding, oral strains of  A. naeslundii genospecies 2 of human ( n = 11) and monkey ( n = 2) origin bound avidly to acidic PRPs but deviated in their relative, although weak, capacities for binding to statherin and oral strains of  A. naeslundii genospecies 1 bound either avidly ( n = 2) or weakly ( n = 4) to acidic PRPs. (ii) In preferential statherin binding,  A. viscosus strains from rat or hamster plaque ( n = 6) and a case of human actinomycosis bound statherin avidly and preferentially.	bind
15968	10	5546	7	10	NULL	NULL	NULL	actinomycosis 	Organism	human	bind		avidly;;preferentially			statherin	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7224_s_108	11705891	(i) In preferential acidic-PRP binding, oral strains of  A. naeslundii genospecies 2 of human ( n = 11) and monkey ( n = 2) origin bound avidly to acidic PRPs but deviated in their relative, although weak, capacities for binding to statherin and oral strains of  A. naeslundii genospecies 1 bound either avidly ( n = 2) or weakly ( n = 4) to acidic PRPs. (ii) In preferential statherin binding,  A. viscosus strains from rat or hamster plaque ( n = 6) and a case of human actinomycosis bound statherin avidly and preferentially.	bind
16611	1	5547	6	10	NULL	NULL	NULL	ArgR1	GP		bind					target DNA sequence	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_18_6059_s_261	15342575	(i) Integrity of the DBDs of both ArgR1 and ArgR2 was necessary for arginine repression, so we conclude that both ArgR proteins bind to target DNA sequences.	bind
16614	2	5547	6	10	NULL	NULL	NULL	ArgR2	GP		bind					target DNA sequence	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_18_6059_s_261	15342575	(i) Integrity of the DBDs of both ArgR1 and ArgR2 was necessary for arginine repression, so we conclude that both ArgR proteins bind to target DNA sequences.	bind
16617	3	5547	6	10	NULL	NULL	NULL	ArgR1	GP	integrity of	is necessary for			DBD		arginine	AminoAcid	repression of 			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_18_6059_s_261	15342575	(i) Integrity of the DBDs of both ArgR1 and ArgR2 was necessary for arginine repression, so we conclude that both ArgR proteins bind to target DNA sequences.	bind
19667	4	5547	6	10	NULL	NULL	NULL	ArgR2	GP	integrity of	is necessary for			DBD		arginine	AminoAcid	repression of			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_18_6059_s_261	15342575	(i) Integrity of the DBDs of both ArgR1 and ArgR2 was necessary for arginine repression, so we conclude that both ArgR proteins bind to target DNA sequences.	bind
19668	5	5547	6	10	NULL	NULL	NULL	statement 3	Process		is simultaneous with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_18_6059_s_261	15342575	(i) Integrity of the DBDs of both ArgR1 and ArgR2 was necessary for arginine repression, so we conclude that both ArgR proteins bind to target DNA sequences.	bind
15970	1	5547	7	10	NULL	NULL	NULL	ArgR1	GP		bind					target DNA sequence	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_18_6059_s_261	15342575	(i) Integrity of the DBDs of both ArgR1 and ArgR2 was necessary for arginine repression, so we conclude that both ArgR proteins bind to target DNA sequences.	bind
15971	2	5547	7	10	NULL	NULL	NULL	ArgR1	GP	Integrity of	is necessary for			DBD		arginine	AminoAcid	repression of			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_18_6059_s_261	15342575	(i) Integrity of the DBDs of both ArgR1 and ArgR2 was necessary for arginine repression, so we conclude that both ArgR proteins bind to target DNA sequences.	bind
15972	3	5547	7	10	NULL	NULL	NULL	ArgR2	GP	Integrity of	is necessary for			DBD		arginine	AminoAcid	repression of			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_18_6059_s_261	15342575	(i) Integrity of the DBDs of both ArgR1 and ArgR2 was necessary for arginine repression, so we conclude that both ArgR proteins bind to target DNA sequences.	bind
19759	4	5547	7	10	NULL	NULL	NULL	statement 2	Process		occurs simultaneous with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_18_6059_s_261	15342575	(i) Integrity of the DBDs of both ArgR1 and ArgR2 was necessary for arginine repression, so we conclude that both ArgR proteins bind to target DNA sequences.	bind
53109	5	5547	7	10	NULL	NULL	NULL	ArgR2	GP		bind					target DNA sequence	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_18_6059_s_261	15342575	(i) Integrity of the DBDs of both ArgR1 and ArgR2 was necessary for arginine repression, so we conclude that both ArgR proteins bind to target DNA sequences.	bind
16619	1	5548	6	10	NULL	NULL	NULL	KIF13A	GP		bind					beta1-adaptin	GP		ear domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_103_4_569_s_161	11106728	(I) KIF13A binds to the ear domain of beta1-adaptin.	bind
15973	1	5548	7	10	NULL	NULL	NULL	KIF13A	GP		binds to					beta1-adaptin	GP		ear domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_103_4_569_s_161	11106728	(I) KIF13A binds to the ear domain of beta1-adaptin.	bind
16620	1	5549	6	10	NULL	NULL	NULL	SSBs	NucleicAcid		activate					PARP-1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_53_55117_s_31	15498778	(i) Ku heterodimer does not represent the sole DSBs recognition complex in cell extracts because it was originally pointed out that PARP-1 is activated  in vitro not only by SSBs but also by DSBs ( ) and that purified PARP-1 binds to DSBs with an efficacy higherR than to SSBs ( ,  ) and with an affinity even greater than that of DNA-PK ( ).	bind
16621	2	5549	6	10	NULL	NULL	NULL	DSBs	NucleicAcid		activate					PARP-1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_53_55117_s_31	15498778	(i) Ku heterodimer does not represent the sole DSBs recognition complex in cell extracts because it was originally pointed out that PARP-1 is activated  in vitro not only by SSBs but also by DSBs ( ) and that purified PARP-1 binds to DSBs with an efficacy higherR than to SSBs ( ,  ) and with an affinity even greater than that of DNA-PK ( ).	bind
16623	3	5549	6	10	NULL	NULL	NULL	PARP-1	GP	purified	bind					DSBs	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_53_55117_s_31	15498778	(i) Ku heterodimer does not represent the sole DSBs recognition complex in cell extracts because it was originally pointed out that PARP-1 is activated  in vitro not only by SSBs but also by DSBs ( ) and that purified PARP-1 binds to DSBs with an efficacy higherR than to SSBs ( ,  ) and with an affinity even greater than that of DNA-PK ( ).	bind
16624	4	5549	6	10	NULL	NULL	NULL	PARP-1	GP	purified	bind					SSBs	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_53_55117_s_31	15498778	(i) Ku heterodimer does not represent the sole DSBs recognition complex in cell extracts because it was originally pointed out that PARP-1 is activated  in vitro not only by SSBs but also by DSBs ( ) and that purified PARP-1 binds to DSBs with an efficacy higherR than to SSBs ( ,  ) and with an affinity even greater than that of DNA-PK ( ).	bind
16626	5	5549	6	10	NULL	NULL	NULL	statement 3	Process		is higher than					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_53_55117_s_31	15498778	(i) Ku heterodimer does not represent the sole DSBs recognition complex in cell extracts because it was originally pointed out that PARP-1 is activated  in vitro not only by SSBs but also by DSBs ( ) and that purified PARP-1 binds to DSBs with an efficacy higherR than to SSBs ( ,  ) and with an affinity even greater than that of DNA-PK ( ).	bind
17048	6	5549	6	10	NULL	NULL	NULL	PARP-1	GP	purified	bind					DNA-PK	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_53_55117_s_31	15498778	(i) Ku heterodimer does not represent the sole DSBs recognition complex in cell extracts because it was originally pointed out that PARP-1 is activated  in vitro not only by SSBs but also by DSBs ( ) and that purified PARP-1 binds to DSBs with an efficacy higherR than to SSBs ( ,  ) and with an affinity even greater than that of DNA-PK ( ).	bind
17049	7	5549	6	10	NULL	NULL	NULL	statement 6	Process		has great efficacy than					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_53_55117_s_31	15498778	(i) Ku heterodimer does not represent the sole DSBs recognition complex in cell extracts because it was originally pointed out that PARP-1 is activated  in vitro not only by SSBs but also by DSBs ( ) and that purified PARP-1 binds to DSBs with an efficacy higherR than to SSBs ( ,  ) and with an affinity even greater than that of DNA-PK ( ).	bind
15974	1	5549	7	10	NULL	NULL	NULL	PARP-1	GP		is activated by					SSBs	NucleicAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_53_55117_s_31	15498778	(i) Ku heterodimer does not represent the sole DSBs recognition complex in cell extracts because it was originally pointed out that PARP-1 is activated  in vitro not only by SSBs but also by DSBs ( ) and that purified PARP-1 binds to DSBs with an efficacy higherR than to SSBs ( ,  ) and with an affinity even greater than that of DNA-PK ( ).	bind
15975	2	5549	7	10	NULL	NULL	NULL	PARP-1	GP		is activated by					DSBs	NucleicAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_53_55117_s_31	15498778	(i) Ku heterodimer does not represent the sole DSBs recognition complex in cell extracts because it was originally pointed out that PARP-1 is activated  in vitro not only by SSBs but also by DSBs ( ) and that purified PARP-1 binds to DSBs with an efficacy higherR than to SSBs ( ,  ) and with an affinity even greater than that of DNA-PK ( ).	bind
15976	3	5549	7	10	NULL	NULL	NULL	PARP-1	GP	purified	bind					DSBs	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_53_55117_s_31	15498778	(i) Ku heterodimer does not represent the sole DSBs recognition complex in cell extracts because it was originally pointed out that PARP-1 is activated  in vitro not only by SSBs but also by DSBs ( ) and that purified PARP-1 binds to DSBs with an efficacy higherR than to SSBs ( ,  ) and with an affinity even greater than that of DNA-PK ( ).	bind
15977	4	5549	7	10	NULL	NULL	NULL	PARP-1	GP	purified	bind					SSBs	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_53_55117_s_31	15498778	(i) Ku heterodimer does not represent the sole DSBs recognition complex in cell extracts because it was originally pointed out that PARP-1 is activated  in vitro not only by SSBs but also by DSBs ( ) and that purified PARP-1 binds to DSBs with an efficacy higherR than to SSBs ( ,  ) and with an affinity even greater than that of DNA-PK ( ).	bind
15978	5	5549	7	10	NULL	NULL	NULL	PARP-1	GP	purified	bind					DNA-PK	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_53_55117_s_31	15498778	(i) Ku heterodimer does not represent the sole DSBs recognition complex in cell extracts because it was originally pointed out that PARP-1 is activated  in vitro not only by SSBs but also by DSBs ( ) and that purified PARP-1 binds to DSBs with an efficacy higherR than to SSBs ( ,  ) and with an affinity even greater than that of DNA-PK ( ).	bind
15979	6	5549	7	10	NULL	NULL	NULL	statement 3	Process		has  greater efficacy than					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_53_55117_s_31	15498778	(i) Ku heterodimer does not represent the sole DSBs recognition complex in cell extracts because it was originally pointed out that PARP-1 is activated  in vitro not only by SSBs but also by DSBs ( ) and that purified PARP-1 binds to DSBs with an efficacy higherR than to SSBs ( ,  ) and with an affinity even greater than that of DNA-PK ( ).	bind
15980	7	5549	7	10	NULL	NULL	NULL	statement 3	Process		greater affinity than					statement 5	Process	 			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_53_55117_s_31	15498778	(i) Ku heterodimer does not represent the sole DSBs recognition complex in cell extracts because it was originally pointed out that PARP-1 is activated  in vitro not only by SSBs but also by DSBs ( ) and that purified PARP-1 binds to DSBs with an efficacy higherR than to SSBs ( ,  ) and with an affinity even greater than that of DNA-PK ( ).	bind
16628	1	5550	6	10	NULL	NULL	NULL	LPS	Chemical		induces					c-Rel	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5523_s_228	9710636	(i) LPS induces more c-Rel, and in 1B4.	bind
15982	1	5550	7	10	NULL	NULL	NULL	 LPS	Chemical		induce					c-Rel	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5523_s_228	9710636	(i) LPS induces more c-Rel, and in 1B4.	bind
16631	1	5551	6	10	NULL	NULL	NULL	m-UBR1	GP		bind					Arg	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_22_8255_s_38	14585983	(I) m-UBR1 and m-UBR2 bind to Arg (type 1) and Phe (type  2) destabilizing N-terminal residues but not to the other tested N-terminal residues.	bind
16633	2	5551	6	10	NULL	NULL	NULL	m-UBR1	GP		bind					Phe	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_22_8255_s_38	14585983	(I) m-UBR1 and m-UBR2 bind to Arg (type 1) and Phe (type  2) destabilizing N-terminal residues but not to the other tested N-terminal residues.	bind
16635	3	5551	6	10	NULL	NULL	NULL	m-UBR2	GP		bind					Arg	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_22_8255_s_38	14585983	(I) m-UBR1 and m-UBR2 bind to Arg (type 1) and Phe (type  2) destabilizing N-terminal residues but not to the other tested N-terminal residues.	bind
16637	4	5551	6	10	NULL	NULL	NULL	m-UBR2	GP		bind					Phe	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_22_8255_s_38	14585983	(I) m-UBR1 and m-UBR2 bind to Arg (type 1) and Phe (type  2) destabilizing N-terminal residues but not to the other tested N-terminal residues.	bind
16638	5	5551	6	10	NULL	NULL	NULL	statement 1	Process		destabilizes								N-terminal residues		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_22_8255_s_38	14585983	(I) m-UBR1 and m-UBR2 bind to Arg (type 1) and Phe (type  2) destabilizing N-terminal residues but not to the other tested N-terminal residues.	bind
16639	6	5551	6	10	NULL	NULL	NULL	statement 2	Process		destabilizes								N-terminal residues		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_22_8255_s_38	14585983	(I) m-UBR1 and m-UBR2 bind to Arg (type 1) and Phe (type  2) destabilizing N-terminal residues but not to the other tested N-terminal residues.	bind
16640	7	5551	6	10	NULL	NULL	NULL	statement 3	Process		destabilizes								N-terminal residues		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_22_8255_s_38	14585983	(I) m-UBR1 and m-UBR2 bind to Arg (type 1) and Phe (type  2) destabilizing N-terminal residues but not to the other tested N-terminal residues.	bind
16641	8	5551	6	10	NULL	NULL	NULL	statement 4	Process		destabilizes								N-terminal residues		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_22_8255_s_38	14585983	(I) m-UBR1 and m-UBR2 bind to Arg (type 1) and Phe (type  2) destabilizing N-terminal residues but not to the other tested N-terminal residues.	bind
15984	1	5551	7	10	NULL	NULL	NULL	m-UBR1	GP		bind					Arg	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_22_8255_s_38	14585983	(I) m-UBR1 and m-UBR2 bind to Arg (type 1) and Phe (type  2) destabilizing N-terminal residues but not to the other tested N-terminal residues.	bind
15985	2	5551	7	10	NULL	NULL	NULL	m-UBR1	GP		bind					Phe	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_22_8255_s_38	14585983	(I) m-UBR1 and m-UBR2 bind to Arg (type 1) and Phe (type  2) destabilizing N-terminal residues but not to the other tested N-terminal residues.	bind
15986	3	5551	7	10	NULL	NULL	NULL	m-UBR2	GP		bind					Arg	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_22_8255_s_38	14585983	(I) m-UBR1 and m-UBR2 bind to Arg (type 1) and Phe (type  2) destabilizing N-terminal residues but not to the other tested N-terminal residues.	bind
15987	4	5551	7	10	NULL	NULL	NULL	m-UBR2	GP		bind					Phe	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_22_8255_s_38	14585983	(I) m-UBR1 and m-UBR2 bind to Arg (type 1) and Phe (type  2) destabilizing N-terminal residues but not to the other tested N-terminal residues.	bind
15988	5	5551	7	10	NULL	NULL	NULL	statement 1	Process		destabilize								N-terminal residues		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_22_8255_s_38	14585983	(I) m-UBR1 and m-UBR2 bind to Arg (type 1) and Phe (type  2) destabilizing N-terminal residues but not to the other tested N-terminal residues.	bind
15989	6	5551	7	10	NULL	NULL	NULL	statement 2	Process		destabilize								N-terminal residues		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_22_8255_s_38	14585983	(I) m-UBR1 and m-UBR2 bind to Arg (type 1) and Phe (type  2) destabilizing N-terminal residues but not to the other tested N-terminal residues.	bind
15990	7	5551	7	10	NULL	NULL	NULL	statement 3	Process		destabilize								N-terminal residues		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_22_8255_s_38	14585983	(I) m-UBR1 and m-UBR2 bind to Arg (type 1) and Phe (type  2) destabilizing N-terminal residues but not to the other tested N-terminal residues.	bind
15991	8	5551	7	10	NULL	NULL	NULL	statement 4	Process		destabilize								N-terminal residues		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_22_8255_s_38	14585983	(I) m-UBR1 and m-UBR2 bind to Arg (type 1) and Phe (type  2) destabilizing N-terminal residues but not to the other tested N-terminal residues.	bind
16643	1	5552	6	10	NULL	NULL	NULL	CRP	GP	purified	bind		directly			traJ	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_5_1616_s_204	12591879	(i) Mobility shift experiments demonstrated that there was direct binding of CRP to the  traJ promoter region; (ii) DNase I footprint experiments showed that binding of purified CRP to a fragment carrying the  traJ promoter region provided protection against DNase I activity; and (iii) targeted mutagenesis of the putative CRP binding sites in the  traJ promoter region reduced the activation of TraJ under starvation conditions.	bind
16644	2	5552	6	10	NULL	NULL	NULL	statement 1	Process		provides protection against					DNase I activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_5_1616_s_204	12591879	(i) Mobility shift experiments demonstrated that there was direct binding of CRP to the  traJ promoter region; (ii) DNase I footprint experiments showed that binding of purified CRP to a fragment carrying the  traJ promoter region provided protection against DNase I activity; and (iii) targeted mutagenesis of the putative CRP binding sites in the  traJ promoter region reduced the activation of TraJ under starvation conditions.	bind
16645	3	5552	6	10	NULL	NULL	NULL	traJ	GP	targeted mutagenesis of;;putative	reduced				CRP binding sites of the promoter	TraJ	GP	activation of 			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_5_1616_s_204	12591879	(i) Mobility shift experiments demonstrated that there was direct binding of CRP to the  traJ promoter region; (ii) DNase I footprint experiments showed that binding of purified CRP to a fragment carrying the  traJ promoter region provided protection against DNase I activity; and (iii) targeted mutagenesis of the putative CRP binding sites in the  traJ promoter region reduced the activation of TraJ under starvation conditions.	bind
16646	4	5552	6	10	NULL	NULL	NULL	statement 3	Process		occurs under					starvation conditions	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_5_1616_s_204	12591879	(i) Mobility shift experiments demonstrated that there was direct binding of CRP to the  traJ promoter region; (ii) DNase I footprint experiments showed that binding of purified CRP to a fragment carrying the  traJ promoter region provided protection against DNase I activity; and (iii) targeted mutagenesis of the putative CRP binding sites in the  traJ promoter region reduced the activation of TraJ under starvation conditions.	bind
15992	1	5552	7	10	NULL	NULL	NULL	CRP	GP	purified	bind		directly			traJ	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_5_1616_s_204	12591879	(i) Mobility shift experiments demonstrated that there was direct binding of CRP to the  traJ promoter region; (ii) DNase I footprint experiments showed that binding of purified CRP to a fragment carrying the  traJ promoter region provided protection against DNase I activity; and (iii) targeted mutagenesis of the putative CRP binding sites in the  traJ promoter region reduced the activation of TraJ under starvation conditions.	bind
15994	3	5552	7	10	NULL	NULL	NULL	traJ fragment	GP		is protected against				promoter	DNase I	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_5_1616_s_204	12591879	(i) Mobility shift experiments demonstrated that there was direct binding of CRP to the  traJ promoter region; (ii) DNase I footprint experiments showed that binding of purified CRP to a fragment carrying the  traJ promoter region provided protection against DNase I activity; and (iii) targeted mutagenesis of the putative CRP binding sites in the  traJ promoter region reduced the activation of TraJ under starvation conditions.	bind
15995	4	5552	7	10	NULL	NULL	NULL	 traJ	GP	 targeted mutagenesis of;;putataive	reduced				CRP site in the promoter	TraJ	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_5_1616_s_204	12591879	(i) Mobility shift experiments demonstrated that there was direct binding of CRP to the  traJ promoter region; (ii) DNase I footprint experiments showed that binding of purified CRP to a fragment carrying the  traJ promoter region provided protection against DNase I activity; and (iii) targeted mutagenesis of the putative CRP binding sites in the  traJ promoter region reduced the activation of TraJ under starvation conditions.	bind
44811	5	5552	7	10	NULL	NULL	NULL	statement 4	Process		occurs under					starvation condition	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_5_1616_s_204	12591879	(i) Mobility shift experiments demonstrated that there was direct binding of CRP to the  traJ promoter region; (ii) DNase I footprint experiments showed that binding of purified CRP to a fragment carrying the  traJ promoter region provided protection against DNase I activity; and (iii) targeted mutagenesis of the putative CRP binding sites in the  traJ promoter region reduced the activation of TraJ under starvation conditions.	bind
16703	1	5553	6	10	NULL	NULL	NULL	Lef	GP		bind					CBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_45_35170_s_155	10906119	(i) Most population of CBP is occupied by beta-catenin because of a much higher levels of beta-catenin than those of Lef/TCF. (ii) High levels of beta-catenin inhibit the binding between Lef and CBP by the association of beta-catenin with Lef and/or CBP and cause the conversion from a Lef-CBP suppression complex to a Lef-beta-catenin-CBP activation complex.	bind
16704	2	5553	6	10	NULL	NULL	NULL	beta-catenin	GP	high levels of	inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_45_35170_s_155	10906119	(i) Most population of CBP is occupied by beta-catenin because of a much higher levels of beta-catenin than those of Lef/TCF. (ii) High levels of beta-catenin inhibit the binding between Lef and CBP by the association of beta-catenin with Lef and/or CBP and cause the conversion from a Lef-CBP suppression complex to a Lef-beta-catenin-CBP activation complex.	bind
16705	3	5553	6	10	NULL	NULL	NULL	statement 1	Process		forms a 					suppression complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_45_35170_s_155	10906119	(i) Most population of CBP is occupied by beta-catenin because of a much higher levels of beta-catenin than those of Lef/TCF. (ii) High levels of beta-catenin inhibit the binding between Lef and CBP by the association of beta-catenin with Lef and/or CBP and cause the conversion from a Lef-CBP suppression complex to a Lef-beta-catenin-CBP activation complex.	bind
16706	4	5553	6	10	NULL	NULL	NULL	beta-catenin	GP		associates with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_45_35170_s_155	10906119	(i) Most population of CBP is occupied by beta-catenin because of a much higher levels of beta-catenin than those of Lef/TCF. (ii) High levels of beta-catenin inhibit the binding between Lef and CBP by the association of beta-catenin with Lef and/or CBP and cause the conversion from a Lef-CBP suppression complex to a Lef-beta-catenin-CBP activation complex.	bind
16707	5	5553	6	10	NULL	NULL	NULL	statement 4	Process		forms a 					Lef-beta-catenin-CBP activation complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_45_35170_s_155	10906119	(i) Most population of CBP is occupied by beta-catenin because of a much higher levels of beta-catenin than those of Lef/TCF. (ii) High levels of beta-catenin inhibit the binding between Lef and CBP by the association of beta-catenin with Lef and/or CBP and cause the conversion from a Lef-CBP suppression complex to a Lef-beta-catenin-CBP activation complex.	bind
44847	6	5553	6	10	NULL	NULL	NULL	Lef-CBP suppression complex	GP		converts to					Lef-beta-catenin-CBP activation complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_45_35170_s_155	10906119	(i) Most population of CBP is occupied by beta-catenin because of a much higher levels of beta-catenin than those of Lef/TCF. (ii) High levels of beta-catenin inhibit the binding between Lef and CBP by the association of beta-catenin with Lef and/or CBP and cause the conversion from a Lef-CBP suppression complex to a Lef-beta-catenin-CBP activation complex.	bind
15996	1	5553	7	10	NULL	NULL	NULL	Lef 	GP		bind					CBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_45_35170_s_155	10906119	(i) Most population of CBP is occupied by beta-catenin because of a much higher levels of beta-catenin than those of Lef/TCF. (ii) High levels of beta-catenin inhibit the binding between Lef and CBP by the association of beta-catenin with Lef and/or CBP and cause the conversion from a Lef-CBP suppression complex to a Lef-beta-catenin-CBP activation complex.	bind
15997	2	5553	7	10	NULL	NULL	NULL	beta-catenin	GP		associate with					Lef	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_45_35170_s_155	10906119	(i) Most population of CBP is occupied by beta-catenin because of a much higher levels of beta-catenin than those of Lef/TCF. (ii) High levels of beta-catenin inhibit the binding between Lef and CBP by the association of beta-catenin with Lef and/or CBP and cause the conversion from a Lef-CBP suppression complex to a Lef-beta-catenin-CBP activation complex.	bind
15998	3	5553	7	10	NULL	NULL	NULL	beta-catenin	GP		associate with					CBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_45_35170_s_155	10906119	(i) Most population of CBP is occupied by beta-catenin because of a much higher levels of beta-catenin than those of Lef/TCF. (ii) High levels of beta-catenin inhibit the binding between Lef and CBP by the association of beta-catenin with Lef and/or CBP and cause the conversion from a Lef-CBP suppression complex to a Lef-beta-catenin-CBP activation complex.	bind
15999	4	5553	7	10	NULL	NULL	NULL	beta-catenin	GP	high levels of	inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_45_35170_s_155	10906119	(i) Most population of CBP is occupied by beta-catenin because of a much higher levels of beta-catenin than those of Lef/TCF. (ii) High levels of beta-catenin inhibit the binding between Lef and CBP by the association of beta-catenin with Lef and/or CBP and cause the conversion from a Lef-CBP suppression complex to a Lef-beta-catenin-CBP activation complex.	bind
16000	5	5553	7	10	NULL	NULL	NULL	statement 4	Process		occurs by					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_45_35170_s_155	10906119	(i) Most population of CBP is occupied by beta-catenin because of a much higher levels of beta-catenin than those of Lef/TCF. (ii) High levels of beta-catenin inhibit the binding between Lef and CBP by the association of beta-catenin with Lef and/or CBP and cause the conversion from a Lef-CBP suppression complex to a Lef-beta-catenin-CBP activation complex.	bind
16001	6	5553	7	10	NULL	NULL	NULL	statement 4	Process		occurs by					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_45_35170_s_155	10906119	(i) Most population of CBP is occupied by beta-catenin because of a much higher levels of beta-catenin than those of Lef/TCF. (ii) High levels of beta-catenin inhibit the binding between Lef and CBP by the association of beta-catenin with Lef and/or CBP and cause the conversion from a Lef-CBP suppression complex to a Lef-beta-catenin-CBP activation complex.	bind
16002	7	5553	7	10	NULL	NULL	NULL	Lef-CBP suppression complex	GP		converts to					Lef-beta-catenin-CBP activation complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_45_35170_s_155	10906119	(i) Most population of CBP is occupied by beta-catenin because of a much higher levels of beta-catenin than those of Lef/TCF. (ii) High levels of beta-catenin inhibit the binding between Lef and CBP by the association of beta-catenin with Lef and/or CBP and cause the conversion from a Lef-CBP suppression complex to a Lef-beta-catenin-CBP activation complex.	bind
16003	8	5553	7	10	NULL	NULL	NULL	statement 2	Process		cause					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_45_35170_s_155	10906119	(i) Most population of CBP is occupied by beta-catenin because of a much higher levels of beta-catenin than those of Lef/TCF. (ii) High levels of beta-catenin inhibit the binding between Lef and CBP by the association of beta-catenin with Lef and/or CBP and cause the conversion from a Lef-CBP suppression complex to a Lef-beta-catenin-CBP activation complex.	bind
16004	9	5553	7	10	NULL	NULL	NULL	statement 3	Process		cause					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_45_35170_s_155	10906119	(i) Most population of CBP is occupied by beta-catenin because of a much higher levels of beta-catenin than those of Lef/TCF. (ii) High levels of beta-catenin inhibit the binding between Lef and CBP by the association of beta-catenin with Lef and/or CBP and cause the conversion from a Lef-CBP suppression complex to a Lef-beta-catenin-CBP activation complex.	bind
17579	1	5554	6	10	NULL	NULL	NULL	p40	GP		bind					p37	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_10_6303_s_225	9045649	(i) No stable complex with two subunits was formed, although weak interactions could be observed for several pairs of subunits; (ii) the only stable three-subunit core complex was formed with p40, p37, and p36; (iii) p140 and p38 bound only cooperatively to the core complex p40.p37.p36 ( 31).	bind
17580	2	5554	6	10	NULL	NULL	NULL	statement 1	Process		bind					p36	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_10_6303_s_225	9045649	(i) No stable complex with two subunits was formed, although weak interactions could be observed for several pairs of subunits; (ii) the only stable three-subunit core complex was formed with p40, p37, and p36; (iii) p140 and p38 bound only cooperatively to the core complex p40.p37.p36 ( 31).	bind
17581	3	5554	6	10	NULL	NULL	NULL	statement 2	Process		forms a 					three-subunit core complex	GP	stable			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_10_6303_s_225	9045649	(i) No stable complex with two subunits was formed, although weak interactions could be observed for several pairs of subunits; (ii) the only stable three-subunit core complex was formed with p40, p37, and p36; (iii) p140 and p38 bound only cooperatively to the core complex p40.p37.p36 ( 31).	bind
17587	4	5554	6	10	NULL	NULL	NULL	p140	GP		bind					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_10_6303_s_225	9045649	(i) No stable complex with two subunits was formed, although weak interactions could be observed for several pairs of subunits; (ii) the only stable three-subunit core complex was formed with p40, p37, and p36; (iii) p140 and p38 bound only cooperatively to the core complex p40.p37.p36 ( 31).	bind
17588	5	5554	6	10	NULL	NULL	NULL	p38	GP		bind					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_10_6303_s_225	9045649	(i) No stable complex with two subunits was formed, although weak interactions could be observed for several pairs of subunits; (ii) the only stable three-subunit core complex was formed with p40, p37, and p36; (iii) p140 and p38 bound only cooperatively to the core complex p40.p37.p36 ( 31).	bind
17590	6	5554	6	10	NULL	NULL	NULL	statement 4	Process		occurs in cooperation with					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_10_6303_s_225	9045649	(i) No stable complex with two subunits was formed, although weak interactions could be observed for several pairs of subunits; (ii) the only stable three-subunit core complex was formed with p40, p37, and p36; (iii) p140 and p38 bound only cooperatively to the core complex p40.p37.p36 ( 31).	bind
16005	1	5554	7	10	NULL	NULL	NULL	p40	GP		bind					p37	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_10_6303_s_225	9045649	(i) No stable complex with two subunits was formed, although weak interactions could be observed for several pairs of subunits; (ii) the only stable three-subunit core complex was formed with p40, p37, and p36; (iii) p140 and p38 bound only cooperatively to the core complex p40.p37.p36 ( 31).	bind
16006	2	5554	7	10	NULL	NULL	NULL	statement 1	Process		bind					p36	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_10_6303_s_225	9045649	(i) No stable complex with two subunits was formed, although weak interactions could be observed for several pairs of subunits; (ii) the only stable three-subunit core complex was formed with p40, p37, and p36; (iii) p140 and p38 bound only cooperatively to the core complex p40.p37.p36 ( 31).	bind
16007	3	5554	7	10	NULL	NULL	NULL	statement 2	Process		forms					three-subunit  core complex	GP	stable			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_10_6303_s_225	9045649	(i) No stable complex with two subunits was formed, although weak interactions could be observed for several pairs of subunits; (ii) the only stable three-subunit core complex was formed with p40, p37, and p36; (iii) p140 and p38 bound only cooperatively to the core complex p40.p37.p36 ( 31).	bind
16008	4	5554	7	10	NULL	NULL	NULL	p140	GP		bind					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_10_6303_s_225	9045649	(i) No stable complex with two subunits was formed, although weak interactions could be observed for several pairs of subunits; (ii) the only stable three-subunit core complex was formed with p40, p37, and p36; (iii) p140 and p38 bound only cooperatively to the core complex p40.p37.p36 ( 31).	bind
16009	5	5554	7	10	NULL	NULL	NULL	p38	GP		bind					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_10_6303_s_225	9045649	(i) No stable complex with two subunits was formed, although weak interactions could be observed for several pairs of subunits; (ii) the only stable three-subunit core complex was formed with p40, p37, and p36; (iii) p140 and p38 bound only cooperatively to the core complex p40.p37.p36 ( 31).	bind
16010	6	5554	7	10	NULL	NULL	NULL	statement 4	Process		occurs in cooperation with					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_10_6303_s_225	9045649	(i) No stable complex with two subunits was formed, although weak interactions could be observed for several pairs of subunits; (ii) the only stable three-subunit core complex was formed with p40, p37, and p36; (iii) p140 and p38 bound only cooperatively to the core complex p40.p37.p36 ( 31).	bind
17059	1	5555	6	10	NULL	NULL	NULL	OATP-C	GP		is expressed in		only			hepatocytes	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_40_37206_s_26	11483603	(i) OATP-C is expressed only in hepatocytes and binding sites for HNF1 have been shown in the promoters or enhancers of numerous genes expressed exclusively in the liver ( 13,  14); (ii) the phenotype of increased serum bile acid concentrations and a 3-10-fold elevation of serum bilirubin in HNF1alpha-deficient (Tcf1 / ) mice ( 11,  15) is consistent with a reduced function of Oatp4 ( Slc21a6), the liver-specific mouse orthologue of human OATP-C ( SLC21A6).	bind
45644	2	5555	6	10	NULL	NULL	NULL	Oatp4	GP		is					Slc21a6	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_40_37206_s_26	11483603	(i) OATP-C is expressed only in hepatocytes and binding sites for HNF1 have been shown in the promoters or enhancers of numerous genes expressed exclusively in the liver ( 13,  14); (ii) the phenotype of increased serum bile acid concentrations and a 3-10-fold elevation of serum bilirubin in HNF1alpha-deficient (Tcf1 / ) mice ( 11,  15) is consistent with a reduced function of Oatp4 ( Slc21a6), the liver-specific mouse orthologue of human OATP-C ( SLC21A6).	bind
45645	3	5555	6	10	NULL	NULL	NULL	Oatp4	GP	mouse;; liver specific	is orthologous to					OATP-C	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_40_37206_s_26	11483603	(i) OATP-C is expressed only in hepatocytes and binding sites for HNF1 have been shown in the promoters or enhancers of numerous genes expressed exclusively in the liver ( 13,  14); (ii) the phenotype of increased serum bile acid concentrations and a 3-10-fold elevation of serum bilirubin in HNF1alpha-deficient (Tcf1 / ) mice ( 11,  15) is consistent with a reduced function of Oatp4 ( Slc21a6), the liver-specific mouse orthologue of human OATP-C ( SLC21A6).	bind
16262	1	5555	7	10	NULL	NULL	NULL	OATP-C	GP		is expressed in		only			hepatocytes	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_40_37206_s_26	11483603	(i) OATP-C is expressed only in hepatocytes and binding sites for HNF1 have been shown in the promoters or enhancers of numerous genes expressed exclusively in the liver ( 13,  14); (ii) the phenotype of increased serum bile acid concentrations and a 3-10-fold elevation of serum bilirubin in HNF1alpha-deficient (Tcf1 / ) mice ( 11,  15) is consistent with a reduced function of Oatp4 ( Slc21a6), the liver-specific mouse orthologue of human OATP-C ( SLC21A6).	bind
16266	2	5555	7	10	NULL	NULL	NULL	Oatp4 	GP	mouse;;liver-specific	is orthologous to					OATP-C	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_40_37206_s_26	11483603	(i) OATP-C is expressed only in hepatocytes and binding sites for HNF1 have been shown in the promoters or enhancers of numerous genes expressed exclusively in the liver ( 13,  14); (ii) the phenotype of increased serum bile acid concentrations and a 3-10-fold elevation of serum bilirubin in HNF1alpha-deficient (Tcf1 / ) mice ( 11,  15) is consistent with a reduced function of Oatp4 ( Slc21a6), the liver-specific mouse orthologue of human OATP-C ( SLC21A6).	bind
45646	3	5555	7	10	NULL	NULL	NULL	Oatp4 	GP		is					Slc21a6	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_40_37206_s_26	11483603	(i) OATP-C is expressed only in hepatocytes and binding sites for HNF1 have been shown in the promoters or enhancers of numerous genes expressed exclusively in the liver ( 13,  14); (ii) the phenotype of increased serum bile acid concentrations and a 3-10-fold elevation of serum bilirubin in HNF1alpha-deficient (Tcf1 / ) mice ( 11,  15) is consistent with a reduced function of Oatp4 ( Slc21a6), the liver-specific mouse orthologue of human OATP-C ( SLC21A6).	bind
45647	4	5555	7	10	NULL	NULL	NULL	OATP-C	GP		is					SLC21A6	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_40_37206_s_26	11483603	(i) OATP-C is expressed only in hepatocytes and binding sites for HNF1 have been shown in the promoters or enhancers of numerous genes expressed exclusively in the liver ( 13,  14); (ii) the phenotype of increased serum bile acid concentrations and a 3-10-fold elevation of serum bilirubin in HNF1alpha-deficient (Tcf1 / ) mice ( 11,  15) is consistent with a reduced function of Oatp4 ( Slc21a6), the liver-specific mouse orthologue of human OATP-C ( SLC21A6).	bind
17060	1	5559	6	10	NULL	NULL	NULL	p105	GP		resides		exclusively			cytosolic compartment	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	bind
17061	2	5559	6	10	NULL	NULL	NULL	statement 1	Process		is independent of					cellular activation	Process	status of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	bind
17063	4	5559	6	10	NULL	NULL	NULL	p105	GP		inhibits			ankyrin motif-rich carboxyl-terminal domain		nuclear expression	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	bind
17064	5	5559	6	10	NULL	NULL	NULL	p105	GP		inhibits			ankyrin motif-rich carboxyl-terminal domain				DNA binding activity of	amino terminal half		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	bind
17602	6	5559	6	10	NULL	NULL	NULL				undergoes		constitutively	IkappaBalpha-related domain		degradation	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	bind
17605	7	5559	6	10	NULL	NULL	NULL	p105	GP		sequesters		physically			RelA	GP				NULL	cytoplasm	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	bind
17608	8	5559	6	10	NULL	NULL	NULL	IkappaBalpha	GP		sequesters		physically			RelA	GP				NULL	cytoplasm	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	bind
17719	9	5559	6	10	NULL	NULL	NULL	p105 gene	GP	inducible	contain							functional		NF-kappaB binding sites	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	bind
17720	10	5559	6	10	NULL	NULL	NULL	IkappaBalpha gene	GP	inducible	contain							functional		NF-kappaB-binding site	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	bind
53117	11	5559	6	10	NULL	NULL	NULL	statement 6	Process		generates					NF-kappaB	GP		p50 DNA binding subunit		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	bind
16034	1	5559	7	10	NULL	NULL	NULL	p105	GP		resides		exclusively			cytosolic compartment	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	bind
16036	2	5559	7	10	NULL	NULL	NULL	statement 1	Process		is independent of					cellular activation	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	bind
16038	3	5559	7	10	NULL	NULL	NULL	p105	GP		inhibits			ankyrin motif-rich carboxyl-terminal domain 		 nuclear expression	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	bind
16042	4	5559	7	10	NULL	NULL	NULL	p105	GP		inhibits			ankyrin motif-rich carboxyl-terminal domain 				DNA binding activity of	half of amino-terminal		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	bind
16045	5	5559	7	10	NULL	NULL	NULL				undergoes		constitutively	IkappaBalpha-related domain		degradation	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	bind
16048	6	5559	7	10	NULL	NULL	NULL	 p105	GP		sequesters		physically			RelA	GP				NULL	cytoplasmic compartment 	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	bind
16049	7	5559	7	10	NULL	NULL	NULL	IkappaBalpha	GP		sequesters		physically			RelA	GP				NULL	cytoplasmic compartment 	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	bind
16050	8	5559	7	10	NULL	NULL	NULL	p105 gene	GP	inducible  	contain							functional	NF-kappaB binding sites		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	bind
16051	9	5559	7	10	NULL	NULL	NULL	IkappaBalpha gene	GP	inducible 	contain							functional	NF-kappaB binding sites		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	bind
53118	10	5559	7	10	NULL	NULL	NULL	statement 5	Process		generates					NF-kappaB	GP		p50 DNA binding subunit		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	bind
17609	1	5560	6	10	NULL	NULL	NULL	VWF	GP	purified	bind					platelets	OrganismPart	human			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_8_4699_s_239	16373331	(i) Peptides derived from these regions inhibited ristocetin-induced binding of purified VWF to human platelets ( ), (ii) stepwise N-terminal deletions in the aa 1204 - 1271 region of a recombinant VWF fragment comprising the A1 domain (aa 1204 - 1496) resulted in stepwise increased ristocetin-induced binding to human platelets ( ); (iii) Ala mutations in the N-terminal flanking region of the A1 domain (aa 1260 - 1271) in full-length VWF resulted in an increased ristocetin-induced binding to human platelets ( ); (iv) deletions in the aa 1222 - 1271 region in full-length VWF in which an additional R1308A mutation was added resulted in an increased ristocetin-induced or even spontaneous binding to human platelets when compared with the R1308A VWF point mutant ( ); (v) specific  O-linked glycosylation in the aa 1248 - 1256 region negatively modulated the binding to human platelets as demonstrated using glycosylphosphatidylinositol COS-7 cell-anchored FLAG-tagged VWF A1 domains ( ).	bind
17610	2	5560	6	10	NULL	NULL	NULL	statement 1	Process		is induced by					ristocetin	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_8_4699_s_239	16373331	(i) Peptides derived from these regions inhibited ristocetin-induced binding of purified VWF to human platelets ( ), (ii) stepwise N-terminal deletions in the aa 1204 - 1271 region of a recombinant VWF fragment comprising the A1 domain (aa 1204 - 1496) resulted in stepwise increased ristocetin-induced binding to human platelets ( ); (iii) Ala mutations in the N-terminal flanking region of the A1 domain (aa 1260 - 1271) in full-length VWF resulted in an increased ristocetin-induced binding to human platelets ( ); (iv) deletions in the aa 1222 - 1271 region in full-length VWF in which an additional R1308A mutation was added resulted in an increased ristocetin-induced or even spontaneous binding to human platelets when compared with the R1308A VWF point mutant ( ); (v) specific  O-linked glycosylation in the aa 1248 - 1256 region negatively modulated the binding to human platelets as demonstrated using glycosylphosphatidylinositol COS-7 cell-anchored FLAG-tagged VWF A1 domains ( ).	bind
17625	3	5560	6	10	NULL	NULL	NULL	VWF fragment	GP	N-terminal deletion;;recombinant	increases			aa 1204 - 1271		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_8_4699_s_239	16373331	(i) Peptides derived from these regions inhibited ristocetin-induced binding of purified VWF to human platelets ( ), (ii) stepwise N-terminal deletions in the aa 1204 - 1271 region of a recombinant VWF fragment comprising the A1 domain (aa 1204 - 1496) resulted in stepwise increased ristocetin-induced binding to human platelets ( ); (iii) Ala mutations in the N-terminal flanking region of the A1 domain (aa 1260 - 1271) in full-length VWF resulted in an increased ristocetin-induced binding to human platelets ( ); (iv) deletions in the aa 1222 - 1271 region in full-length VWF in which an additional R1308A mutation was added resulted in an increased ristocetin-induced or even spontaneous binding to human platelets when compared with the R1308A VWF point mutant ( ); (v) specific  O-linked glycosylation in the aa 1248 - 1256 region negatively modulated the binding to human platelets as demonstrated using glycosylphosphatidylinositol COS-7 cell-anchored FLAG-tagged VWF A1 domains ( ).	bind
17660	4	5560	6	10	NULL	NULL	NULL	VWF	GP	full length;;mutant	increases			Ala		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_8_4699_s_239	16373331	(i) Peptides derived from these regions inhibited ristocetin-induced binding of purified VWF to human platelets ( ), (ii) stepwise N-terminal deletions in the aa 1204 - 1271 region of a recombinant VWF fragment comprising the A1 domain (aa 1204 - 1496) resulted in stepwise increased ristocetin-induced binding to human platelets ( ); (iii) Ala mutations in the N-terminal flanking region of the A1 domain (aa 1260 - 1271) in full-length VWF resulted in an increased ristocetin-induced binding to human platelets ( ); (iv) deletions in the aa 1222 - 1271 region in full-length VWF in which an additional R1308A mutation was added resulted in an increased ristocetin-induced or even spontaneous binding to human platelets when compared with the R1308A VWF point mutant ( ); (v) specific  O-linked glycosylation in the aa 1248 - 1256 region negatively modulated the binding to human platelets as demonstrated using glycosylphosphatidylinositol COS-7 cell-anchored FLAG-tagged VWF A1 domains ( ).	bind
17661	5	5560	6	10	NULL	NULL	NULL	VWF	GP	deletion mutant;;full-length	increases			aa1222-1271;;R1308A		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_8_4699_s_239	16373331	(i) Peptides derived from these regions inhibited ristocetin-induced binding of purified VWF to human platelets ( ), (ii) stepwise N-terminal deletions in the aa 1204 - 1271 region of a recombinant VWF fragment comprising the A1 domain (aa 1204 - 1496) resulted in stepwise increased ristocetin-induced binding to human platelets ( ); (iii) Ala mutations in the N-terminal flanking region of the A1 domain (aa 1260 - 1271) in full-length VWF resulted in an increased ristocetin-induced binding to human platelets ( ); (iv) deletions in the aa 1222 - 1271 region in full-length VWF in which an additional R1308A mutation was added resulted in an increased ristocetin-induced or even spontaneous binding to human platelets when compared with the R1308A VWF point mutant ( ); (v) specific  O-linked glycosylation in the aa 1248 - 1256 region negatively modulated the binding to human platelets as demonstrated using glycosylphosphatidylinositol COS-7 cell-anchored FLAG-tagged VWF A1 domains ( ).	bind
17662	6	5560	6	10	NULL	NULL	NULL	VWF	GP	glycosylated	negatively modulates			aa 1248-1256		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_8_4699_s_239	16373331	(i) Peptides derived from these regions inhibited ristocetin-induced binding of purified VWF to human platelets ( ), (ii) stepwise N-terminal deletions in the aa 1204 - 1271 region of a recombinant VWF fragment comprising the A1 domain (aa 1204 - 1496) resulted in stepwise increased ristocetin-induced binding to human platelets ( ); (iii) Ala mutations in the N-terminal flanking region of the A1 domain (aa 1260 - 1271) in full-length VWF resulted in an increased ristocetin-induced binding to human platelets ( ); (iv) deletions in the aa 1222 - 1271 region in full-length VWF in which an additional R1308A mutation was added resulted in an increased ristocetin-induced or even spontaneous binding to human platelets when compared with the R1308A VWF point mutant ( ); (v) specific  O-linked glycosylation in the aa 1248 - 1256 region negatively modulated the binding to human platelets as demonstrated using glycosylphosphatidylinositol COS-7 cell-anchored FLAG-tagged VWF A1 domains ( ).	bind
16103	1	5560	7	10	NULL	NULL	NULL	VWF	GP	purified 	bind					platelets	OrganismPart	human			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_8_4699_s_239	16373331	(i) Peptides derived from these regions inhibited ristocetin-induced binding of purified VWF to human platelets ( ), (ii) stepwise N-terminal deletions in the aa 1204 - 1271 region of a recombinant VWF fragment comprising the A1 domain (aa 1204 - 1496) resulted in stepwise increased ristocetin-induced binding to human platelets ( ); (iii) Ala mutations in the N-terminal flanking region of the A1 domain (aa 1260 - 1271) in full-length VWF resulted in an increased ristocetin-induced binding to human platelets ( ); (iv) deletions in the aa 1222 - 1271 region in full-length VWF in which an additional R1308A mutation was added resulted in an increased ristocetin-induced or even spontaneous binding to human platelets when compared with the R1308A VWF point mutant ( ); (v) specific  O-linked glycosylation in the aa 1248 - 1256 region negatively modulated the binding to human platelets as demonstrated using glycosylphosphatidylinositol COS-7 cell-anchored FLAG-tagged VWF A1 domains ( ).	bind
16105	2	5560	7	10	NULL	NULL	NULL	ristocetin	Chemical		induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_8_4699_s_239	16373331	(i) Peptides derived from these regions inhibited ristocetin-induced binding of purified VWF to human platelets ( ), (ii) stepwise N-terminal deletions in the aa 1204 - 1271 region of a recombinant VWF fragment comprising the A1 domain (aa 1204 - 1496) resulted in stepwise increased ristocetin-induced binding to human platelets ( ); (iii) Ala mutations in the N-terminal flanking region of the A1 domain (aa 1260 - 1271) in full-length VWF resulted in an increased ristocetin-induced binding to human platelets ( ); (iv) deletions in the aa 1222 - 1271 region in full-length VWF in which an additional R1308A mutation was added resulted in an increased ristocetin-induced or even spontaneous binding to human platelets when compared with the R1308A VWF point mutant ( ); (v) specific  O-linked glycosylation in the aa 1248 - 1256 region negatively modulated the binding to human platelets as demonstrated using glycosylphosphatidylinositol COS-7 cell-anchored FLAG-tagged VWF A1 domains ( ).	bind
16117	3	5560	7	10	NULL	NULL	NULL	VWF fragment	GP	deletion of;;recombinant	increase			N-terminal aa 1204 - 1271 		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_8_4699_s_239	16373331	(i) Peptides derived from these regions inhibited ristocetin-induced binding of purified VWF to human platelets ( ), (ii) stepwise N-terminal deletions in the aa 1204 - 1271 region of a recombinant VWF fragment comprising the A1 domain (aa 1204 - 1496) resulted in stepwise increased ristocetin-induced binding to human platelets ( ); (iii) Ala mutations in the N-terminal flanking region of the A1 domain (aa 1260 - 1271) in full-length VWF resulted in an increased ristocetin-induced binding to human platelets ( ); (iv) deletions in the aa 1222 - 1271 region in full-length VWF in which an additional R1308A mutation was added resulted in an increased ristocetin-induced or even spontaneous binding to human platelets when compared with the R1308A VWF point mutant ( ); (v) specific  O-linked glycosylation in the aa 1248 - 1256 region negatively modulated the binding to human platelets as demonstrated using glycosylphosphatidylinositol COS-7 cell-anchored FLAG-tagged VWF A1 domains ( ).	bind
16119	4	5560	7	10	NULL	NULL	NULL	VWF fragment	GP		comprise								 A1 domain aa 1204 - 1496		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_8_4699_s_239	16373331	(i) Peptides derived from these regions inhibited ristocetin-induced binding of purified VWF to human platelets ( ), (ii) stepwise N-terminal deletions in the aa 1204 - 1271 region of a recombinant VWF fragment comprising the A1 domain (aa 1204 - 1496) resulted in stepwise increased ristocetin-induced binding to human platelets ( ); (iii) Ala mutations in the N-terminal flanking region of the A1 domain (aa 1260 - 1271) in full-length VWF resulted in an increased ristocetin-induced binding to human platelets ( ); (iv) deletions in the aa 1222 - 1271 region in full-length VWF in which an additional R1308A mutation was added resulted in an increased ristocetin-induced or even spontaneous binding to human platelets when compared with the R1308A VWF point mutant ( ); (v) specific  O-linked glycosylation in the aa 1248 - 1256 region negatively modulated the binding to human platelets as demonstrated using glycosylphosphatidylinositol COS-7 cell-anchored FLAG-tagged VWF A1 domains ( ).	bind
16123	5	5560	7	10	NULL	NULL	NULL	Ala	AminoAcid	mutations of	increase			N- terminal flanking region of the A1 domain aa 1260 - 1271		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_8_4699_s_239	16373331	(i) Peptides derived from these regions inhibited ristocetin-induced binding of purified VWF to human platelets ( ), (ii) stepwise N-terminal deletions in the aa 1204 - 1271 region of a recombinant VWF fragment comprising the A1 domain (aa 1204 - 1496) resulted in stepwise increased ristocetin-induced binding to human platelets ( ); (iii) Ala mutations in the N-terminal flanking region of the A1 domain (aa 1260 - 1271) in full-length VWF resulted in an increased ristocetin-induced binding to human platelets ( ); (iv) deletions in the aa 1222 - 1271 region in full-length VWF in which an additional R1308A mutation was added resulted in an increased ristocetin-induced or even spontaneous binding to human platelets when compared with the R1308A VWF point mutant ( ); (v) specific  O-linked glycosylation in the aa 1248 - 1256 region negatively modulated the binding to human platelets as demonstrated using glycosylphosphatidylinositol COS-7 cell-anchored FLAG-tagged VWF A1 domains ( ).	bind
16126	6	5560	7	10	NULL	NULL	NULL	VWF	GP	deletion mutant;;full-length	increase			aa 1222 - 1271		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_8_4699_s_239	16373331	(i) Peptides derived from these regions inhibited ristocetin-induced binding of purified VWF to human platelets ( ), (ii) stepwise N-terminal deletions in the aa 1204 - 1271 region of a recombinant VWF fragment comprising the A1 domain (aa 1204 - 1496) resulted in stepwise increased ristocetin-induced binding to human platelets ( ); (iii) Ala mutations in the N-terminal flanking region of the A1 domain (aa 1260 - 1271) in full-length VWF resulted in an increased ristocetin-induced binding to human platelets ( ); (iv) deletions in the aa 1222 - 1271 region in full-length VWF in which an additional R1308A mutation was added resulted in an increased ristocetin-induced or even spontaneous binding to human platelets when compared with the R1308A VWF point mutant ( ); (v) specific  O-linked glycosylation in the aa 1248 - 1256 region negatively modulated the binding to human platelets as demonstrated using glycosylphosphatidylinositol COS-7 cell-anchored FLAG-tagged VWF A1 domains ( ).	bind
16132	7	5560	7	10	NULL	NULL	NULL	VWF	GP	deletion mutant;;full-length	result in			aa1222-1271		statement 2	Process	spontaneous			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_8_4699_s_239	16373331	(i) Peptides derived from these regions inhibited ristocetin-induced binding of purified VWF to human platelets ( ), (ii) stepwise N-terminal deletions in the aa 1204 - 1271 region of a recombinant VWF fragment comprising the A1 domain (aa 1204 - 1496) resulted in stepwise increased ristocetin-induced binding to human platelets ( ); (iii) Ala mutations in the N-terminal flanking region of the A1 domain (aa 1260 - 1271) in full-length VWF resulted in an increased ristocetin-induced binding to human platelets ( ); (iv) deletions in the aa 1222 - 1271 region in full-length VWF in which an additional R1308A mutation was added resulted in an increased ristocetin-induced or even spontaneous binding to human platelets when compared with the R1308A VWF point mutant ( ); (v) specific  O-linked glycosylation in the aa 1248 - 1256 region negatively modulated the binding to human platelets as demonstrated using glycosylphosphatidylinositol COS-7 cell-anchored FLAG-tagged VWF A1 domains ( ).	bind
16133	8	5560	7	10	NULL	NULL	NULL	statement 6	Process	additional mutation to	increase			R1308A		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_8_4699_s_239	16373331	(i) Peptides derived from these regions inhibited ristocetin-induced binding of purified VWF to human platelets ( ), (ii) stepwise N-terminal deletions in the aa 1204 - 1271 region of a recombinant VWF fragment comprising the A1 domain (aa 1204 - 1496) resulted in stepwise increased ristocetin-induced binding to human platelets ( ); (iii) Ala mutations in the N-terminal flanking region of the A1 domain (aa 1260 - 1271) in full-length VWF resulted in an increased ristocetin-induced binding to human platelets ( ); (iv) deletions in the aa 1222 - 1271 region in full-length VWF in which an additional R1308A mutation was added resulted in an increased ristocetin-induced or even spontaneous binding to human platelets when compared with the R1308A VWF point mutant ( ); (v) specific  O-linked glycosylation in the aa 1248 - 1256 region negatively modulated the binding to human platelets as demonstrated using glycosylphosphatidylinositol COS-7 cell-anchored FLAG-tagged VWF A1 domains ( ).	bind
16136	9	5560	7	10	NULL	NULL	NULL	statement 7	Process	additional mutation to	increase			R1308A		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_8_4699_s_239	16373331	(i) Peptides derived from these regions inhibited ristocetin-induced binding of purified VWF to human platelets ( ), (ii) stepwise N-terminal deletions in the aa 1204 - 1271 region of a recombinant VWF fragment comprising the A1 domain (aa 1204 - 1496) resulted in stepwise increased ristocetin-induced binding to human platelets ( ); (iii) Ala mutations in the N-terminal flanking region of the A1 domain (aa 1260 - 1271) in full-length VWF resulted in an increased ristocetin-induced binding to human platelets ( ); (iv) deletions in the aa 1222 - 1271 region in full-length VWF in which an additional R1308A mutation was added resulted in an increased ristocetin-induced or even spontaneous binding to human platelets when compared with the R1308A VWF point mutant ( ); (v) specific  O-linked glycosylation in the aa 1248 - 1256 region negatively modulated the binding to human platelets as demonstrated using glycosylphosphatidylinositol COS-7 cell-anchored FLAG-tagged VWF A1 domains ( ).	bind
16137	10	5560	7	10	NULL	NULL	NULL	VWF	GP	point mutant	increase			R1308A		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_8_4699_s_239	16373331	(i) Peptides derived from these regions inhibited ristocetin-induced binding of purified VWF to human platelets ( ), (ii) stepwise N-terminal deletions in the aa 1204 - 1271 region of a recombinant VWF fragment comprising the A1 domain (aa 1204 - 1496) resulted in stepwise increased ristocetin-induced binding to human platelets ( ); (iii) Ala mutations in the N-terminal flanking region of the A1 domain (aa 1260 - 1271) in full-length VWF resulted in an increased ristocetin-induced binding to human platelets ( ); (iv) deletions in the aa 1222 - 1271 region in full-length VWF in which an additional R1308A mutation was added resulted in an increased ristocetin-induced or even spontaneous binding to human platelets when compared with the R1308A VWF point mutant ( ); (v) specific  O-linked glycosylation in the aa 1248 - 1256 region negatively modulated the binding to human platelets as demonstrated using glycosylphosphatidylinositol COS-7 cell-anchored FLAG-tagged VWF A1 domains ( ).	bind
16138	11	5560	7	10	NULL	NULL	NULL	statement 8	Process		is increased 					statement 10	Process	compared with			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_8_4699_s_239	16373331	(i) Peptides derived from these regions inhibited ristocetin-induced binding of purified VWF to human platelets ( ), (ii) stepwise N-terminal deletions in the aa 1204 - 1271 region of a recombinant VWF fragment comprising the A1 domain (aa 1204 - 1496) resulted in stepwise increased ristocetin-induced binding to human platelets ( ); (iii) Ala mutations in the N-terminal flanking region of the A1 domain (aa 1260 - 1271) in full-length VWF resulted in an increased ristocetin-induced binding to human platelets ( ); (iv) deletions in the aa 1222 - 1271 region in full-length VWF in which an additional R1308A mutation was added resulted in an increased ristocetin-induced or even spontaneous binding to human platelets when compared with the R1308A VWF point mutant ( ); (v) specific  O-linked glycosylation in the aa 1248 - 1256 region negatively modulated the binding to human platelets as demonstrated using glycosylphosphatidylinositol COS-7 cell-anchored FLAG-tagged VWF A1 domains ( ).	bind
16139	12	5560	7	10	NULL	NULL	NULL	statement 9	Process		is increased					statement 10	Process	compared with			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_8_4699_s_239	16373331	(i) Peptides derived from these regions inhibited ristocetin-induced binding of purified VWF to human platelets ( ), (ii) stepwise N-terminal deletions in the aa 1204 - 1271 region of a recombinant VWF fragment comprising the A1 domain (aa 1204 - 1496) resulted in stepwise increased ristocetin-induced binding to human platelets ( ); (iii) Ala mutations in the N-terminal flanking region of the A1 domain (aa 1260 - 1271) in full-length VWF resulted in an increased ristocetin-induced binding to human platelets ( ); (iv) deletions in the aa 1222 - 1271 region in full-length VWF in which an additional R1308A mutation was added resulted in an increased ristocetin-induced or even spontaneous binding to human platelets when compared with the R1308A VWF point mutant ( ); (v) specific  O-linked glycosylation in the aa 1248 - 1256 region negatively modulated the binding to human platelets as demonstrated using glycosylphosphatidylinositol COS-7 cell-anchored FLAG-tagged VWF A1 domains ( ).	bind
16140	13	5560	7	10	NULL	NULL	NULL			O-linked glycosylation	negatively modulates			aa 1248 - 1256		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_8_4699_s_239	16373331	(i) Peptides derived from these regions inhibited ristocetin-induced binding of purified VWF to human platelets ( ), (ii) stepwise N-terminal deletions in the aa 1204 - 1271 region of a recombinant VWF fragment comprising the A1 domain (aa 1204 - 1496) resulted in stepwise increased ristocetin-induced binding to human platelets ( ); (iii) Ala mutations in the N-terminal flanking region of the A1 domain (aa 1260 - 1271) in full-length VWF resulted in an increased ristocetin-induced binding to human platelets ( ); (iv) deletions in the aa 1222 - 1271 region in full-length VWF in which an additional R1308A mutation was added resulted in an increased ristocetin-induced or even spontaneous binding to human platelets when compared with the R1308A VWF point mutant ( ); (v) specific  O-linked glycosylation in the aa 1248 - 1256 region negatively modulated the binding to human platelets as demonstrated using glycosylphosphatidylinositol COS-7 cell-anchored FLAG-tagged VWF A1 domains ( ).	bind
17065	1	5561	6	10	NULL	NULL	NULL	86 kDa protein	GP	phosphorylated	bind					F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainres_757_1_24_s_178	9200495	(i) Phospho- and dephospho-86 kDa protein bind to F-actin, with apparent dissociation constants of  Kd 280 nM and  Kd 690 nM, respectively.	bind
17066	2	5561	6	10	NULL	NULL	NULL	86 kDa protein	GP	dephosphorylated	bind					F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainres_757_1_24_s_178	9200495	(i) Phospho- and dephospho-86 kDa protein bind to F-actin, with apparent dissociation constants of  Kd 280 nM and  Kd 690 nM, respectively.	bind
16142	1	5561	7	10	NULL	NULL	NULL	86 kDa protein	GP	phosphorylated	bind					F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainres_757_1_24_s_178	9200495	(i) Phospho- and dephospho-86 kDa protein bind to F-actin, with apparent dissociation constants of  Kd 280 nM and  Kd 690 nM, respectively.	bind
16143	2	5561	7	10	NULL	NULL	NULL	86 kDa protein	GP	dephosphorylated	bind					F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainres_757_1_24_s_178	9200495	(i) Phospho- and dephospho-86 kDa protein bind to F-actin, with apparent dissociation constants of  Kd 280 nM and  Kd 690 nM, respectively.	bind
17067	1	5563	6	10	NULL	NULL	NULL	Rtp-YFP	GP		bind							endogenous		ter sites	NULL	strain IRN424	NULL	NULL	NULL	NULL	gw70_jbacteriol_185_4_1326_s_167	12562803	(I) Position of Rtp-YFP  bound to endogenous  ter sites (strain IRN424).	bind
16144	1	5563	7	10	NULL	NULL	NULL	Rtp-YFP	GP		bind							endogenous		ter sites	NULL	strain IRN424	NULL	NULL	NULL	NULL	gw70_jbacteriol_185_4_1326_s_167	12562803	(I) Position of Rtp-YFP  bound to endogenous  ter sites (strain IRN424).	bind
17069	1	5565	6	10	NULL	NULL	NULL	PPARalpha	GP		bind							natural		PPRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25252_s_6	9312141	(i) PPARgamma in combination with either RXRalpha or RXRgamma binds more strongly than PPARalpha or PPARbeta to all natural PPREs tested.	bind
17070	2	5565	6	10	NULL	NULL	NULL	PPARbeta	GP		bind							natural		PPRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25252_s_6	9312141	(i) PPARgamma in combination with either RXRalpha or RXRgamma binds more strongly than PPARalpha or PPARbeta to all natural PPREs tested.	bind
17074	3	5565	6	10	NULL	NULL	NULL	PPARgamma	GP		bind							natural		PPRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25252_s_6	9312141	(i) PPARgamma in combination with either RXRalpha or RXRgamma binds more strongly than PPARalpha or PPARbeta to all natural PPREs tested.	bind
17075	4	5565	6	10	NULL	NULL	NULL	RXRalpha	GP		bind							natural		PPRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25252_s_6	9312141	(i) PPARgamma in combination with either RXRalpha or RXRgamma binds more strongly than PPARalpha or PPARbeta to all natural PPREs tested.	bind
17076	6	5565	6	10	NULL	NULL	NULL	statement 5	Process		is stronger than					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25252_s_6	9312141	(i) PPARgamma in combination with either RXRalpha or RXRgamma binds more strongly than PPARalpha or PPARbeta to all natural PPREs tested.	bind
17077	7	5565	6	10	NULL	NULL	NULL	statement 5	Process		is stronger than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25252_s_6	9312141	(i) PPARgamma in combination with either RXRalpha or RXRgamma binds more strongly than PPARalpha or PPARbeta to all natural PPREs tested.	bind
17078	10	5565	6	10	NULL	NULL	NULL	statement 9	Process		is stronger than					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25252_s_6	9312141	(i) PPARgamma in combination with either RXRalpha or RXRgamma binds more strongly than PPARalpha or PPARbeta to all natural PPREs tested.	bind
17079	11	5565	6	10	NULL	NULL	NULL	statement 9	Process		is stronger than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25252_s_6	9312141	(i) PPARgamma in combination with either RXRalpha or RXRgamma binds more strongly than PPARalpha or PPARbeta to all natural PPREs tested.	bind
53122	5	5565	6	10	NULL	NULL	NULL	statement 3	Process		in combination with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25252_s_6	9312141	(i) PPARgamma in combination with either RXRalpha or RXRgamma binds more strongly than PPARalpha or PPARbeta to all natural PPREs tested.	bind
53123	8	5565	6	10	NULL	NULL	NULL	RXRgamma	GP		bind							natural		PPRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25252_s_6	9312141	(i) PPARgamma in combination with either RXRalpha or RXRgamma binds more strongly than PPARalpha or PPARbeta to all natural PPREs tested.	bind
53124	9	5565	6	10	NULL	NULL	NULL	statement 3	Process		in combination with					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25252_s_6	9312141	(i) PPARgamma in combination with either RXRalpha or RXRgamma binds more strongly than PPARalpha or PPARbeta to all natural PPREs tested.	bind
16147	1	5565	7	10	NULL	NULL	NULL	PPARgamma	GP		bind							natural		PPRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25252_s_6	9312141	(i) PPARgamma in combination with either RXRalpha or RXRgamma binds more strongly than PPARalpha or PPARbeta to all natural PPREs tested.	bind
16148	2	5565	7	10	NULL	NULL	NULL	RXRgamma	GP		bind							natural		PPRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25252_s_6	9312141	(i) PPARgamma in combination with either RXRalpha or RXRgamma binds more strongly than PPARalpha or PPARbeta to all natural PPREs tested.	bind
16149	3	5565	7	10	NULL	NULL	NULL	PPARalpha	GP		bind							natural		PPRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25252_s_6	9312141	(i) PPARgamma in combination with either RXRalpha or RXRgamma binds more strongly than PPARalpha or PPARbeta to all natural PPREs tested.	bind
16150	4	5565	7	10	NULL	NULL	NULL	PPARbeta	GP		bind							natural		PPRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25252_s_6	9312141	(i) PPARgamma in combination with either RXRalpha or RXRgamma binds more strongly than PPARalpha or PPARbeta to all natural PPREs tested.	bind
16151	8	5565	7	10	NULL	NULL	NULL	statement 6	Process		is stronger than					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25252_s_6	9312141	(i) PPARgamma in combination with either RXRalpha or RXRgamma binds more strongly than PPARalpha or PPARbeta to all natural PPREs tested.	bind
16152	9	5565	7	10	NULL	NULL	NULL	statement 6	Process		is stronger than					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25252_s_6	9312141	(i) PPARgamma in combination with either RXRalpha or RXRgamma binds more strongly than PPARalpha or PPARbeta to all natural PPREs tested.	bind
16153	10	5565	7	10	NULL	NULL	NULL	statement 7	Process		is stronger than					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25252_s_6	9312141	(i) PPARgamma in combination with either RXRalpha or RXRgamma binds more strongly than PPARalpha or PPARbeta to all natural PPREs tested.	bind
16154	11	5565	7	10	NULL	NULL	NULL	statement 7	Process		is stronger than					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25252_s_6	9312141	(i) PPARgamma in combination with either RXRalpha or RXRgamma binds more strongly than PPARalpha or PPARbeta to all natural PPREs tested.	bind
53119	5	5565	7	10	NULL	NULL	NULL	RXRalpha	GP		bind							natural		PPRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25252_s_6	9312141	(i) PPARgamma in combination with either RXRalpha or RXRgamma binds more strongly than PPARalpha or PPARbeta to all natural PPREs tested.	bind
53120	6	5565	7	10	NULL	NULL	NULL	statement 1	Process		in combination with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25252_s_6	9312141	(i) PPARgamma in combination with either RXRalpha or RXRgamma binds more strongly than PPARalpha or PPARbeta to all natural PPREs tested.	bind
53121	7	5565	7	10	NULL	NULL	NULL	statement 1	Process		in combination with					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25252_s_6	9312141	(i) PPARgamma in combination with either RXRalpha or RXRgamma binds more strongly than PPARalpha or PPARbeta to all natural PPREs tested.	bind
17080	1	5566	6	10	NULL	NULL	NULL	Sp1	GP		bind					FP-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_49_40650_s_290	16216869	(I) promoter activity nor Sp1 binding to FP-2 by PPARgamma.	bind
16155	1	5566	7	10	NULL	NULL	NULL	 Sp1	GP		bind					FP-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_49_40650_s_290	16216869	(I) promoter activity nor Sp1 binding to FP-2 by PPARgamma.	bind
17083	1	5568	6	10	NULL	NULL	NULL	Rab1B	GP	wt	bind					REP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_23_20379_s_242	11389151	(i) Rab1B(wt) binds to REP and is di-geranylgeranylated exclusively by GGTase II. (ii) Rab1B(Y78D) cannot bind REP and therefore fails to undergo prenylation.	bind
17084	2	5568	6	10	NULL	NULL	NULL	GGTase II	GP		di-geranylgeranylate		exclusively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_23_20379_s_242	11389151	(i) Rab1B(wt) binds to REP and is di-geranylgeranylated exclusively by GGTase II. (ii) Rab1B(Y78D) cannot bind REP and therefore fails to undergo prenylation.	bind
17085	3	5568	6	10	NULL	NULL	NULL	Rab1B	GP		does not bind			Y78D		REP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_23_20379_s_242	11389151	(i) Rab1B(wt) binds to REP and is di-geranylgeranylated exclusively by GGTase II. (ii) Rab1B(Y78D) cannot bind REP and therefore fails to undergo prenylation.	bind
17086	4	5568	6	10	NULL	NULL	NULL	Rab1B	GP		does not undergo			Y78D		prenylation	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_23_20379_s_242	11389151	(i) Rab1B(wt) binds to REP and is di-geranylgeranylated exclusively by GGTase II. (ii) Rab1B(Y78D) cannot bind REP and therefore fails to undergo prenylation.	bind
17087	5	5568	6	10	NULL	NULL	NULL	statement 4	Process		occurs due to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_23_20379_s_242	11389151	(i) Rab1B(wt) binds to REP and is di-geranylgeranylated exclusively by GGTase II. (ii) Rab1B(Y78D) cannot bind REP and therefore fails to undergo prenylation.	bind
16157	1	5568	7	10	NULL	NULL	NULL	Rab1B	GP	wt	bind					REP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_23_20379_s_242	11389151	(i) Rab1B(wt) binds to REP and is di-geranylgeranylated exclusively by GGTase II. (ii) Rab1B(Y78D) cannot bind REP and therefore fails to undergo prenylation.	bind
16158	2	5568	7	10	NULL	NULL	NULL	GGTase II	GP		di-geranylgeranylates		exclusively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_23_20379_s_242	11389151	(i) Rab1B(wt) binds to REP and is di-geranylgeranylated exclusively by GGTase II. (ii) Rab1B(Y78D) cannot bind REP and therefore fails to undergo prenylation.	bind
16159	3	5568	7	10	NULL	NULL	NULL	Rab1B	GP		does not bind			Y78D		REP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_23_20379_s_242	11389151	(i) Rab1B(wt) binds to REP and is di-geranylgeranylated exclusively by GGTase II. (ii) Rab1B(Y78D) cannot bind REP and therefore fails to undergo prenylation.	bind
16160	4	5568	7	10	NULL	NULL	NULL	statement 3	Process		fails to undergo					prenylation	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_23_20379_s_242	11389151	(i) Rab1B(wt) binds to REP and is di-geranylgeranylated exclusively by GGTase II. (ii) Rab1B(Y78D) cannot bind REP and therefore fails to undergo prenylation.	bind
17663	1	5571	6	10	NULL	NULL	NULL	SCR 8-14 	GP		inhibits		partially			SCR 8-15/PspC	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_10_5604_s_216	12228288	(i) SCR 13 and SCR 15 may come together to form the strongest PspC binding site, and this protein may partially displace the weaker binding SCR 8-14 (containing only SCR 13) from PspC. (ii) There may be an additional binding site for SCR 15 on PspC, which is distinct from the SCR 13 binding site, explaining why SCR 8-14 is only partially inhibitory of SCR 8-15/PspC binding.	bind
17721	2	5571	6	10	NULL	NULL	NULL	SCR 13	GP		bind					SCR 15	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_10_5604_s_216	12228288	(i) SCR 13 and SCR 15 may come together to form the strongest PspC binding site, and this protein may partially displace the weaker binding SCR 8-14 (containing only SCR 13) from PspC. (ii) There may be an additional binding site for SCR 15 on PspC, which is distinct from the SCR 13 binding site, explaining why SCR 8-14 is only partially inhibitory of SCR 8-15/PspC binding.	bind
17722	3	5571	6	10	NULL	NULL	NULL	statement 2	Process		forms							strongest		PspC binding site	NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_10_5604_s_216	12228288	(i) SCR 13 and SCR 15 may come together to form the strongest PspC binding site, and this protein may partially displace the weaker binding SCR 8-14 (containing only SCR 13) from PspC. (ii) There may be an additional binding site for SCR 15 on PspC, which is distinct from the SCR 13 binding site, explaining why SCR 8-14 is only partially inhibitory of SCR 8-15/PspC binding.	bind
17723	4	5571	6	10	NULL	NULL	NULL	SCR 8-14	GP		contains		only			SCR 13	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_10_5604_s_216	12228288	(i) SCR 13 and SCR 15 may come together to form the strongest PspC binding site, and this protein may partially displace the weaker binding SCR 8-14 (containing only SCR 13) from PspC. (ii) There may be an additional binding site for SCR 15 on PspC, which is distinct from the SCR 13 binding site, explaining why SCR 8-14 is only partially inhibitory of SCR 8-15/PspC binding.	bind
17724	5	5571	6	10	NULL	NULL	NULL	statement 4	Process		bind		weakly			PspC	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_10_5604_s_216	12228288	(i) SCR 13 and SCR 15 may come together to form the strongest PspC binding site, and this protein may partially displace the weaker binding SCR 8-14 (containing only SCR 13) from PspC. (ii) There may be an additional binding site for SCR 15 on PspC, which is distinct from the SCR 13 binding site, explaining why SCR 8-14 is only partially inhibitory of SCR 8-15/PspC binding.	bind
17725	6	5571	6	10	NULL	NULL	NULL	statement 3	Process		displace		may;; partially			statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_10_5604_s_216	12228288	(i) SCR 13 and SCR 15 may come together to form the strongest PspC binding site, and this protein may partially displace the weaker binding SCR 8-14 (containing only SCR 13) from PspC. (ii) There may be an additional binding site for SCR 15 on PspC, which is distinct from the SCR 13 binding site, explaining why SCR 8-14 is only partially inhibitory of SCR 8-15/PspC binding.	bind
16161	1	5571	7	10	NULL	NULL	NULL	SCR 13 	GP		bind 					SCR 15	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_10_5604_s_216	12228288	(i) SCR 13 and SCR 15 may come together to form the strongest PspC binding site, and this protein may partially displace the weaker binding SCR 8-14 (containing only SCR 13) from PspC. (ii) There may be an additional binding site for SCR 15 on PspC, which is distinct from the SCR 13 binding site, explaining why SCR 8-14 is only partially inhibitory of SCR 8-15/PspC binding.	bind
16162	2	5571	7	10	NULL	NULL	NULL	statement 1	Process		forms							strongest	PspC binding site		NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_10_5604_s_216	12228288	(i) SCR 13 and SCR 15 may come together to form the strongest PspC binding site, and this protein may partially displace the weaker binding SCR 8-14 (containing only SCR 13) from PspC. (ii) There may be an additional binding site for SCR 15 on PspC, which is distinct from the SCR 13 binding site, explaining why SCR 8-14 is only partially inhibitory of SCR 8-15/PspC binding.	bind
16163	4	5571	7	10	NULL	NULL	NULL	statement 2	Process		displace		may;;partially			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_10_5604_s_216	12228288	(i) SCR 13 and SCR 15 may come together to form the strongest PspC binding site, and this protein may partially displace the weaker binding SCR 8-14 (containing only SCR 13) from PspC. (ii) There may be an additional binding site for SCR 15 on PspC, which is distinct from the SCR 13 binding site, explaining why SCR 8-14 is only partially inhibitory of SCR 8-15/PspC binding.	bind
16164	5	5571	7	10	NULL	NULL	NULL	statement 3	Process		contains only					SCR 13	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_10_5604_s_216	12228288	(i) SCR 13 and SCR 15 may come together to form the strongest PspC binding site, and this protein may partially displace the weaker binding SCR 8-14 (containing only SCR 13) from PspC. (ii) There may be an additional binding site for SCR 15 on PspC, which is distinct from the SCR 13 binding site, explaining why SCR 8-14 is only partially inhibitory of SCR 8-15/PspC binding.	bind
16165	6	5571	7	10	NULL	NULL	NULL	SCR 8-15	GP		bind					PspC	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_10_5604_s_216	12228288	(i) SCR 13 and SCR 15 may come together to form the strongest PspC binding site, and this protein may partially displace the weaker binding SCR 8-14 (containing only SCR 13) from PspC. (ii) There may be an additional binding site for SCR 15 on PspC, which is distinct from the SCR 13 binding site, explaining why SCR 8-14 is only partially inhibitory of SCR 8-15/PspC binding.	bind
16166	7	5571	7	10	NULL	NULL	NULL	SCR 8-14	GP		inhibits		partially			SCR 8-15/PspC	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_10_5604_s_216	12228288	(i) SCR 13 and SCR 15 may come together to form the strongest PspC binding site, and this protein may partially displace the weaker binding SCR 8-14 (containing only SCR 13) from PspC. (ii) There may be an additional binding site for SCR 15 on PspC, which is distinct from the SCR 13 binding site, explaining why SCR 8-14 is only partially inhibitory of SCR 8-15/PspC binding.	bind
44934	3	5571	7	10	NULL	NULL	NULL	SCR 8-14	GP		bind		weakly			PspC	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_10_5604_s_216	12228288	(i) SCR 13 and SCR 15 may come together to form the strongest PspC binding site, and this protein may partially displace the weaker binding SCR 8-14 (containing only SCR 13) from PspC. (ii) There may be an additional binding site for SCR 15 on PspC, which is distinct from the SCR 13 binding site, explaining why SCR 8-14 is only partially inhibitory of SCR 8-15/PspC binding.	bind
17157	1	5572	6	10	NULL	NULL	NULL	Actin	GP		bind					Kelch	GP	nonphosphorylated			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_156_4_703_s_86	11854310	(I) showed that actin was bound only to the nonphosphorylated form of Kelch.	bind
16167	1	5572	7	10	NULL	NULL	NULL	actin	GP		bind					Kelch	GP	nonphosphorylated 			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_156_4_703_s_86	11854310	(I) showed that actin was bound only to the nonphosphorylated form of Kelch.	bind
17158	1	5573	6	10	NULL	NULL	NULL	TFIIB	GP		bind		robustly			Sp1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_19_6958_s_286	12972613	(I) site in DAPA revealed robust binding of TFIIB to the Sp1	bind
16168	1	5573	7	10	NULL	NULL	NULL	 TFIIB	GP		bind		robustly			Sp1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_19_6958_s_286	12972613	(I) site in DAPA revealed robust binding of TFIIB to the Sp1	bind
17159	1	5574	6	10	NULL	NULL	NULL	Stat5B	GP		bind					insulin receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15985_s_253	10821852	(i) Stat5B binds to the insulin receptor, as shown by a yeast two-hybrid assay.	bind
16170	1	5574	7	10	NULL	NULL	NULL	 Stat5B	GP		binds to					insulin receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15985_s_253	10821852	(i) Stat5B binds to the insulin receptor, as shown by a yeast two-hybrid assay.	bind
20034	1	5575	6	10	NULL	NULL	NULL	poly L-proline	AminoAcid		does not bind					type II prolyl 4-hydroxylase tetramer	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_2_306_s_177	9889187	(I) subunit by glutamate and glutamine, respectively, in the alpha(II) subunit appears to explain most of the lack of poly(L-proline) binding of the type II prolyl 4-hydroxylase tetramer.	bind
16171	1	5575	7	10	NULL	NULL	NULL	poly L-proline	AminoAcid		does not bind					type II prolyl 4-hydroxylase tetramer	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_2_306_s_177	9889187	(I) subunit by glutamate and glutamine, respectively, in the alpha(II) subunit appears to explain most of the lack of poly(L-proline) binding of the type II prolyl 4-hydroxylase tetramer.	bind
17160	1	5577	6	10	NULL	NULL	NULL	At-P4H-1	GP		bind			Lys270		2-oxoglutarate	Chemical		C-5 carboxyl group		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_26_23965_s_130	11976332	(I) subunit, the At-P4H-1 Lys270 corresponds to the lysine that binds the C-5 carboxyl group of 2-oxoglutarate, and the At-P4H-1 Arg278 corresponds to the fifth critical residue, a histidine or an arginine depending on the species, which is probably involved in both the binding of the C-1 carboxyl group of 2-oxoglutarate to the Fe2+ atom and the decarboxylation of this cosubstrate ( 12,  26,  34).	bind
17167	2	5577	6	10	NULL	NULL	NULL	2-oxoglutarate	Chemical		bind			C-1 carboxyl group		Fe+2 atom	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_26_23965_s_130	11976332	(I) subunit, the At-P4H-1 Lys270 corresponds to the lysine that binds the C-5 carboxyl group of 2-oxoglutarate, and the At-P4H-1 Arg278 corresponds to the fifth critical residue, a histidine or an arginine depending on the species, which is probably involved in both the binding of the C-1 carboxyl group of 2-oxoglutarate to the Fe2+ atom and the decarboxylation of this cosubstrate ( 12,  26,  34).	bind
17187	3	5577	6	10	NULL	NULL	NULL	At-P4H-1	GP		is involved in			Arg278		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_26_23965_s_130	11976332	(I) subunit, the At-P4H-1 Lys270 corresponds to the lysine that binds the C-5 carboxyl group of 2-oxoglutarate, and the At-P4H-1 Arg278 corresponds to the fifth critical residue, a histidine or an arginine depending on the species, which is probably involved in both the binding of the C-1 carboxyl group of 2-oxoglutarate to the Fe2+ atom and the decarboxylation of this cosubstrate ( 12,  26,  34).	bind
17188	4	5577	6	10	NULL	NULL	NULL	At-P4H-1	GP		is involved in			Arg278		cosubstrate	Chemical	decarboxylation of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_26_23965_s_130	11976332	(I) subunit, the At-P4H-1 Lys270 corresponds to the lysine that binds the C-5 carboxyl group of 2-oxoglutarate, and the At-P4H-1 Arg278 corresponds to the fifth critical residue, a histidine or an arginine depending on the species, which is probably involved in both the binding of the C-1 carboxyl group of 2-oxoglutarate to the Fe2+ atom and the decarboxylation of this cosubstrate ( 12,  26,  34).	bind
16172	1	5577	7	10	NULL	NULL	NULL	At-P4H-1 	GP		binds			Lys270		2-oxoglutarate	Chemical		C-5 carboxyl group		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_26_23965_s_130	11976332	(I) subunit, the At-P4H-1 Lys270 corresponds to the lysine that binds the C-5 carboxyl group of 2-oxoglutarate, and the At-P4H-1 Arg278 corresponds to the fifth critical residue, a histidine or an arginine depending on the species, which is probably involved in both the binding of the C-1 carboxyl group of 2-oxoglutarate to the Fe2+ atom and the decarboxylation of this cosubstrate ( 12,  26,  34).	bind
16173	2	5577	7	10	NULL	NULL	NULL	2-oxoglutarate	Chemical		binds			C-1 carboxyl group		Fe2+ atom	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_26_23965_s_130	11976332	(I) subunit, the At-P4H-1 Lys270 corresponds to the lysine that binds the C-5 carboxyl group of 2-oxoglutarate, and the At-P4H-1 Arg278 corresponds to the fifth critical residue, a histidine or an arginine depending on the species, which is probably involved in both the binding of the C-1 carboxyl group of 2-oxoglutarate to the Fe2+ atom and the decarboxylation of this cosubstrate ( 12,  26,  34).	bind
16174	3	5577	7	10	NULL	NULL	NULL	At-P4H-1	GP		is involved in			Arg278		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_26_23965_s_130	11976332	(I) subunit, the At-P4H-1 Lys270 corresponds to the lysine that binds the C-5 carboxyl group of 2-oxoglutarate, and the At-P4H-1 Arg278 corresponds to the fifth critical residue, a histidine or an arginine depending on the species, which is probably involved in both the binding of the C-1 carboxyl group of 2-oxoglutarate to the Fe2+ atom and the decarboxylation of this cosubstrate ( 12,  26,  34).	bind
16175	4	5577	7	10	NULL	NULL	NULL	At-P4H-1	GP		is involved in			Arg278		cosubstrate	Chemical	decarboxylation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_26_23965_s_130	11976332	(I) subunit, the At-P4H-1 Lys270 corresponds to the lysine that binds the C-5 carboxyl group of 2-oxoglutarate, and the At-P4H-1 Arg278 corresponds to the fifth critical residue, a histidine or an arginine depending on the species, which is probably involved in both the binding of the C-1 carboxyl group of 2-oxoglutarate to the Fe2+ atom and the decarboxylation of this cosubstrate ( 12,  26,  34).	bind
17189	1	5578	6	10	NULL	NULL	NULL	Sxl protein	GP		bind					msl-2 mRNA	NucleicAcid			3'UTR	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_3018_s_264	10082569	(i) Sxl protein binds to the 3' UTRs of  msl-2 and  Sxl mRNAs in vivo.	bind
17190	2	5578	6	10	NULL	NULL	NULL	Sxl protein	GP		bind					Sxl mRNA	NucleicAcid			3' UTR	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_3018_s_264	10082569	(i) Sxl protein binds to the 3' UTRs of  msl-2 and  Sxl mRNAs in vivo.	bind
16176	1	5578	7	10	NULL	NULL	NULL	Sxl protein	GP		bind					 msl-2 mRNA	NucleicAcid			 3' UTRs	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_3018_s_264	10082569	(i) Sxl protein binds to the 3' UTRs of  msl-2 and  Sxl mRNAs in vivo.	bind
16177	2	5578	7	10	NULL	NULL	NULL	Sxl protein	GP		bind					Sxl mRNA	NucleicAcid			 3' UTRs	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_3018_s_264	10082569	(i) Sxl protein binds to the 3' UTRs of  msl-2 and  Sxl mRNAs in vivo.	bind
17191	1	5579	6	10	NULL	NULL	NULL	ADR1	GP		bind			TADIV		TFIID components	GP	yeast			NULL	yeast crude extracts	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_10_5861_s_193	9742103	(i) TADIV of ADR1 binds TFIID components from yeast crude extracts; (ii) the ability of derivatives of TADIV to bind TFIID components correlates with TADIV activation potential; (iii) deletion of TADIV from ADR1 severely compromises ADR1 function; (iv) the transcriptional potential of LexA-ADR1-TADIV was more severely compromised than that of other activation domains by a  taf130/145 allele; (v) ADR1 coimmunoprecipitates with either TAFII90 or TBP; and (vi) TFIID appears to be required for ADR1-dependent activation of  ADH2 in vivo, as depletion of yeast cells of TAFII90 prevents  ADH2 derepression.	bind
17664	2	5579	6	10	NULL	NULL	NULL	statement 1	Process		corelates with					TADIV	GP	activation potential of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_10_5861_s_193	9742103	(i) TADIV of ADR1 binds TFIID components from yeast crude extracts; (ii) the ability of derivatives of TADIV to bind TFIID components correlates with TADIV activation potential; (iii) deletion of TADIV from ADR1 severely compromises ADR1 function; (iv) the transcriptional potential of LexA-ADR1-TADIV was more severely compromised than that of other activation domains by a  taf130/145 allele; (v) ADR1 coimmunoprecipitates with either TAFII90 or TBP; and (vi) TFIID appears to be required for ADR1-dependent activation of  ADH2 in vivo, as depletion of yeast cells of TAFII90 prevents  ADH2 derepression.	bind
17665	3	5579	6	10	NULL	NULL	NULL	ADR1	GP	deletion of	compromises		severely	TADIV		ADR1	GP	function of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_10_5861_s_193	9742103	(i) TADIV of ADR1 binds TFIID components from yeast crude extracts; (ii) the ability of derivatives of TADIV to bind TFIID components correlates with TADIV activation potential; (iii) deletion of TADIV from ADR1 severely compromises ADR1 function; (iv) the transcriptional potential of LexA-ADR1-TADIV was more severely compromised than that of other activation domains by a  taf130/145 allele; (v) ADR1 coimmunoprecipitates with either TAFII90 or TBP; and (vi) TFIID appears to be required for ADR1-dependent activation of  ADH2 in vivo, as depletion of yeast cells of TAFII90 prevents  ADH2 derepression.	bind
17666	4	5579	6	10	NULL	NULL	NULL	ADR1	GP		coimmunoprecipates with					TAFII90	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_10_5861_s_193	9742103	(i) TADIV of ADR1 binds TFIID components from yeast crude extracts; (ii) the ability of derivatives of TADIV to bind TFIID components correlates with TADIV activation potential; (iii) deletion of TADIV from ADR1 severely compromises ADR1 function; (iv) the transcriptional potential of LexA-ADR1-TADIV was more severely compromised than that of other activation domains by a  taf130/145 allele; (v) ADR1 coimmunoprecipitates with either TAFII90 or TBP; and (vi) TFIID appears to be required for ADR1-dependent activation of  ADH2 in vivo, as depletion of yeast cells of TAFII90 prevents  ADH2 derepression.	bind
17667	5	5579	6	10	NULL	NULL	NULL	ADR1	GP		coimmunoprecipitates with					TBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_10_5861_s_193	9742103	(i) TADIV of ADR1 binds TFIID components from yeast crude extracts; (ii) the ability of derivatives of TADIV to bind TFIID components correlates with TADIV activation potential; (iii) deletion of TADIV from ADR1 severely compromises ADR1 function; (iv) the transcriptional potential of LexA-ADR1-TADIV was more severely compromised than that of other activation domains by a  taf130/145 allele; (v) ADR1 coimmunoprecipitates with either TAFII90 or TBP; and (vi) TFIID appears to be required for ADR1-dependent activation of  ADH2 in vivo, as depletion of yeast cells of TAFII90 prevents  ADH2 derepression.	bind
17668	6	5579	6	10	NULL	NULL	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_10_5861_s_193	9742103	(i) TADIV of ADR1 binds TFIID components from yeast crude extracts; (ii) the ability of derivatives of TADIV to bind TFIID components correlates with TADIV activation potential; (iii) deletion of TADIV from ADR1 severely compromises ADR1 function; (iv) the transcriptional potential of LexA-ADR1-TADIV was more severely compromised than that of other activation domains by a  taf130/145 allele; (v) ADR1 coimmunoprecipitates with either TAFII90 or TBP; and (vi) TFIID appears to be required for ADR1-dependent activation of  ADH2 in vivo, as depletion of yeast cells of TAFII90 prevents  ADH2 derepression.	bind
17669	7	5579	6	10	NULL	NULL	NULL	ADH2	GP	activation of	is dependent on					ADR1	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_10_5861_s_193	9742103	(i) TADIV of ADR1 binds TFIID components from yeast crude extracts; (ii) the ability of derivatives of TADIV to bind TFIID components correlates with TADIV activation potential; (iii) deletion of TADIV from ADR1 severely compromises ADR1 function; (iv) the transcriptional potential of LexA-ADR1-TADIV was more severely compromised than that of other activation domains by a  taf130/145 allele; (v) ADR1 coimmunoprecipitates with either TAFII90 or TBP; and (vi) TFIID appears to be required for ADR1-dependent activation of  ADH2 in vivo, as depletion of yeast cells of TAFII90 prevents  ADH2 derepression.	bind
17670	8	5579	6	10	NULL	NULL	NULL	TFIID	GP		is required for					statement 7	Process				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_10_5861_s_193	9742103	(i) TADIV of ADR1 binds TFIID components from yeast crude extracts; (ii) the ability of derivatives of TADIV to bind TFIID components correlates with TADIV activation potential; (iii) deletion of TADIV from ADR1 severely compromises ADR1 function; (iv) the transcriptional potential of LexA-ADR1-TADIV was more severely compromised than that of other activation domains by a  taf130/145 allele; (v) ADR1 coimmunoprecipitates with either TAFII90 or TBP; and (vi) TFIID appears to be required for ADR1-dependent activation of  ADH2 in vivo, as depletion of yeast cells of TAFII90 prevents  ADH2 derepression.	bind
17726	9	5579	6	10	NULL	NULL	NULL	TAFII90	GP	depletion of	prevents					ADH2	GP	depression of			NULL	yeast cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_10_5861_s_193	9742103	(i) TADIV of ADR1 binds TFIID components from yeast crude extracts; (ii) the ability of derivatives of TADIV to bind TFIID components correlates with TADIV activation potential; (iii) deletion of TADIV from ADR1 severely compromises ADR1 function; (iv) the transcriptional potential of LexA-ADR1-TADIV was more severely compromised than that of other activation domains by a  taf130/145 allele; (v) ADR1 coimmunoprecipitates with either TAFII90 or TBP; and (vi) TFIID appears to be required for ADR1-dependent activation of  ADH2 in vivo, as depletion of yeast cells of TAFII90 prevents  ADH2 derepression.	bind
16178	1	5579	7	10	NULL	NULL	NULL	ADR1	GP		binds			TADIV		TFIID components	GP				NULL	yeast crude extract	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_10_5861_s_193	9742103	(i) TADIV of ADR1 binds TFIID components from yeast crude extracts; (ii) the ability of derivatives of TADIV to bind TFIID components correlates with TADIV activation potential; (iii) deletion of TADIV from ADR1 severely compromises ADR1 function; (iv) the transcriptional potential of LexA-ADR1-TADIV was more severely compromised than that of other activation domains by a  taf130/145 allele; (v) ADR1 coimmunoprecipitates with either TAFII90 or TBP; and (vi) TFIID appears to be required for ADR1-dependent activation of  ADH2 in vivo, as depletion of yeast cells of TAFII90 prevents  ADH2 derepression.	bind
16179	2	5579	7	10	NULL	NULL	NULL	statement 1	Process		correlates with							activation potential	TADIV 		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_10_5861_s_193	9742103	(i) TADIV of ADR1 binds TFIID components from yeast crude extracts; (ii) the ability of derivatives of TADIV to bind TFIID components correlates with TADIV activation potential; (iii) deletion of TADIV from ADR1 severely compromises ADR1 function; (iv) the transcriptional potential of LexA-ADR1-TADIV was more severely compromised than that of other activation domains by a  taf130/145 allele; (v) ADR1 coimmunoprecipitates with either TAFII90 or TBP; and (vi) TFIID appears to be required for ADR1-dependent activation of  ADH2 in vivo, as depletion of yeast cells of TAFII90 prevents  ADH2 derepression.	bind
16180	3	5579	7	10	NULL	NULL	NULL	ADR1	GP	deletion of	compromise		severely	TADIV 		ADR1	GP	function of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_10_5861_s_193	9742103	(i) TADIV of ADR1 binds TFIID components from yeast crude extracts; (ii) the ability of derivatives of TADIV to bind TFIID components correlates with TADIV activation potential; (iii) deletion of TADIV from ADR1 severely compromises ADR1 function; (iv) the transcriptional potential of LexA-ADR1-TADIV was more severely compromised than that of other activation domains by a  taf130/145 allele; (v) ADR1 coimmunoprecipitates with either TAFII90 or TBP; and (vi) TFIID appears to be required for ADR1-dependent activation of  ADH2 in vivo, as depletion of yeast cells of TAFII90 prevents  ADH2 derepression.	bind
16186	5	5579	7	10	NULL	NULL	NULL	ADR1	GP		\tcoimmunoprecipitates with					TAFII90	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_10_5861_s_193	9742103	(i) TADIV of ADR1 binds TFIID components from yeast crude extracts; (ii) the ability of derivatives of TADIV to bind TFIID components correlates with TADIV activation potential; (iii) deletion of TADIV from ADR1 severely compromises ADR1 function; (iv) the transcriptional potential of LexA-ADR1-TADIV was more severely compromised than that of other activation domains by a  taf130/145 allele; (v) ADR1 coimmunoprecipitates with either TAFII90 or TBP; and (vi) TFIID appears to be required for ADR1-dependent activation of  ADH2 in vivo, as depletion of yeast cells of TAFII90 prevents  ADH2 derepression.	bind
16187	6	5579	7	10	NULL	NULL	NULL	ADR1	GP		\tcoimmunoprecipitates with					TBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_10_5861_s_193	9742103	(i) TADIV of ADR1 binds TFIID components from yeast crude extracts; (ii) the ability of derivatives of TADIV to bind TFIID components correlates with TADIV activation potential; (iii) deletion of TADIV from ADR1 severely compromises ADR1 function; (iv) the transcriptional potential of LexA-ADR1-TADIV was more severely compromised than that of other activation domains by a  taf130/145 allele; (v) ADR1 coimmunoprecipitates with either TAFII90 or TBP; and (vi) TFIID appears to be required for ADR1-dependent activation of  ADH2 in vivo, as depletion of yeast cells of TAFII90 prevents  ADH2 derepression.	bind
16188	7	5579	7	10	NULL	NULL	NULL	ADH2	GP	activation of	is dependent on					ADR1	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_10_5861_s_193	9742103	(i) TADIV of ADR1 binds TFIID components from yeast crude extracts; (ii) the ability of derivatives of TADIV to bind TFIID components correlates with TADIV activation potential; (iii) deletion of TADIV from ADR1 severely compromises ADR1 function; (iv) the transcriptional potential of LexA-ADR1-TADIV was more severely compromised than that of other activation domains by a  taf130/145 allele; (v) ADR1 coimmunoprecipitates with either TAFII90 or TBP; and (vi) TFIID appears to be required for ADR1-dependent activation of  ADH2 in vivo, as depletion of yeast cells of TAFII90 prevents  ADH2 derepression.	bind
16189	8	5579	7	10	NULL	NULL	NULL	TFIID	GP		is required for					statement 7	Process				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_10_5861_s_193	9742103	(i) TADIV of ADR1 binds TFIID components from yeast crude extracts; (ii) the ability of derivatives of TADIV to bind TFIID components correlates with TADIV activation potential; (iii) deletion of TADIV from ADR1 severely compromises ADR1 function; (iv) the transcriptional potential of LexA-ADR1-TADIV was more severely compromised than that of other activation domains by a  taf130/145 allele; (v) ADR1 coimmunoprecipitates with either TAFII90 or TBP; and (vi) TFIID appears to be required for ADR1-dependent activation of  ADH2 in vivo, as depletion of yeast cells of TAFII90 prevents  ADH2 derepression.	bind
16190	9	5579	7	10	NULL	NULL	NULL	TAFII90	GP	depletion of	prevents					ADH2	GP	derepression of			NULL	yeast cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_10_5861_s_193	9742103	(i) TADIV of ADR1 binds TFIID components from yeast crude extracts; (ii) the ability of derivatives of TADIV to bind TFIID components correlates with TADIV activation potential; (iii) deletion of TADIV from ADR1 severely compromises ADR1 function; (iv) the transcriptional potential of LexA-ADR1-TADIV was more severely compromised than that of other activation domains by a  taf130/145 allele; (v) ADR1 coimmunoprecipitates with either TAFII90 or TBP; and (vi) TFIID appears to be required for ADR1-dependent activation of  ADH2 in vivo, as depletion of yeast cells of TAFII90 prevents  ADH2 derepression.	bind
17771	10	5579	7	10	NULL	NULL	NULL	statement 5	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_10_5861_s_193	9742103	(i) TADIV of ADR1 binds TFIID components from yeast crude extracts; (ii) the ability of derivatives of TADIV to bind TFIID components correlates with TADIV activation potential; (iii) deletion of TADIV from ADR1 severely compromises ADR1 function; (iv) the transcriptional potential of LexA-ADR1-TADIV was more severely compromised than that of other activation domains by a  taf130/145 allele; (v) ADR1 coimmunoprecipitates with either TAFII90 or TBP; and (vi) TFIID appears to be required for ADR1-dependent activation of  ADH2 in vivo, as depletion of yeast cells of TAFII90 prevents  ADH2 derepression.	bind
17671	1	5580	6	10	NULL	NULL	NULL	CheY	GP		bind					CheZ	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_13_7357_s_57	8631757	(i) The  CheY(N23D) mutant protein is impaired in its interaction with CheZ,  thus affecting the ability of CheZ to bind and dephosphorylate it; or  (ii) the binding of CheY(N23D) to CheZ is stronger compared to  wild-type CheY, so that most of the CheZ present in the reaction would  be ```sequestered'''  leaving residual CheY(N23D), which would  be dephosphorylated only by spontaneous hydrolysis.	bind
17672	2	5580	6	10	NULL	NULL	NULL	CheY	GP	mutant	affects			N23D		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_13_7357_s_57	8631757	(i) The  CheY(N23D) mutant protein is impaired in its interaction with CheZ,  thus affecting the ability of CheZ to bind and dephosphorylate it; or  (ii) the binding of CheY(N23D) to CheZ is stronger compared to  wild-type CheY, so that most of the CheZ present in the reaction would  be ```sequestered'''  leaving residual CheY(N23D), which would  be dephosphorylated only by spontaneous hydrolysis.	bind
17673	3	5580	6	10	NULL	NULL	NULL	CheZ	GP		dephosphorylate					CheY	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_13_7357_s_57	8631757	(i) The  CheY(N23D) mutant protein is impaired in its interaction with CheZ,  thus affecting the ability of CheZ to bind and dephosphorylate it; or  (ii) the binding of CheY(N23D) to CheZ is stronger compared to  wild-type CheY, so that most of the CheZ present in the reaction would  be ```sequestered'''  leaving residual CheY(N23D), which would  be dephosphorylated only by spontaneous hydrolysis.	bind
17674	4	5580	6	10	NULL	NULL	NULL	CheY	GP	mutant	affects			N23D		statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_13_7357_s_57	8631757	(i) The  CheY(N23D) mutant protein is impaired in its interaction with CheZ,  thus affecting the ability of CheZ to bind and dephosphorylate it; or  (ii) the binding of CheY(N23D) to CheZ is stronger compared to  wild-type CheY, so that most of the CheZ present in the reaction would  be ```sequestered'''  leaving residual CheY(N23D), which would  be dephosphorylated only by spontaneous hydrolysis.	bind
17675	5	5580	6	10	NULL	NULL	NULL	CheY	GP	mutant	bind			N23D		CheZ	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_13_7357_s_57	8631757	(i) The  CheY(N23D) mutant protein is impaired in its interaction with CheZ,  thus affecting the ability of CheZ to bind and dephosphorylate it; or  (ii) the binding of CheY(N23D) to CheZ is stronger compared to  wild-type CheY, so that most of the CheZ present in the reaction would  be ```sequestered'''  leaving residual CheY(N23D), which would  be dephosphorylated only by spontaneous hydrolysis.	bind
17676	6	5580	6	10	NULL	NULL	NULL	CheY	GP	wild type	bind					CheZ	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_13_7357_s_57	8631757	(i) The  CheY(N23D) mutant protein is impaired in its interaction with CheZ,  thus affecting the ability of CheZ to bind and dephosphorylate it; or  (ii) the binding of CheY(N23D) to CheZ is stronger compared to  wild-type CheY, so that most of the CheZ present in the reaction would  be ```sequestered'''  leaving residual CheY(N23D), which would  be dephosphorylated only by spontaneous hydrolysis.	bind
17677	7	5580	6	10	NULL	NULL	NULL	statement 5	Process		is stronger than					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_13_7357_s_57	8631757	(i) The  CheY(N23D) mutant protein is impaired in its interaction with CheZ,  thus affecting the ability of CheZ to bind and dephosphorylate it; or  (ii) the binding of CheY(N23D) to CheZ is stronger compared to  wild-type CheY, so that most of the CheZ present in the reaction would  be ```sequestered'''  leaving residual CheY(N23D), which would  be dephosphorylated only by spontaneous hydrolysis.	bind
20035	8	5580	6	10	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_13_7357_s_57	8631757	(i) The  CheY(N23D) mutant protein is impaired in its interaction with CheZ,  thus affecting the ability of CheZ to bind and dephosphorylate it; or  (ii) the binding of CheY(N23D) to CheZ is stronger compared to  wild-type CheY, so that most of the CheZ present in the reaction would  be ```sequestered'''  leaving residual CheY(N23D), which would  be dephosphorylated only by spontaneous hydrolysis.	bind
16191	1	5580	7	10	NULL	NULL	NULL	CheY	GP	mutant	impairs			N23D		CheZ	GP	interaction of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_13_7357_s_57	8631757	(i) The  CheY(N23D) mutant protein is impaired in its interaction with CheZ,  thus affecting the ability of CheZ to bind and dephosphorylate it; or  (ii) the binding of CheY(N23D) to CheZ is stronger compared to  wild-type CheY, so that most of the CheZ present in the reaction would  be ```sequestered'''  leaving residual CheY(N23D), which would  be dephosphorylated only by spontaneous hydrolysis.	bind
16192	2	5580	7	10	NULL	NULL	NULL	statement 1	Process		affects					CheZ	GP	the binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_13_7357_s_57	8631757	(i) The  CheY(N23D) mutant protein is impaired in its interaction with CheZ,  thus affecting the ability of CheZ to bind and dephosphorylate it; or  (ii) the binding of CheY(N23D) to CheZ is stronger compared to  wild-type CheY, so that most of the CheZ present in the reaction would  be ```sequestered'''  leaving residual CheY(N23D), which would  be dephosphorylated only by spontaneous hydrolysis.	bind
16193	3	5580	7	10	NULL	NULL	NULL	CheZ	GP		dephosphorylates					CheY	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_13_7357_s_57	8631757	(i) The  CheY(N23D) mutant protein is impaired in its interaction with CheZ,  thus affecting the ability of CheZ to bind and dephosphorylate it; or  (ii) the binding of CheY(N23D) to CheZ is stronger compared to  wild-type CheY, so that most of the CheZ present in the reaction would  be ```sequestered'''  leaving residual CheY(N23D), which would  be dephosphorylated only by spontaneous hydrolysis.	bind
16196	8	5580	7	10	NULL	NULL	NULL	statement 5	Process		leaves behind					CheY	GP	 residual	N23D		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_13_7357_s_57	8631757	(i) The  CheY(N23D) mutant protein is impaired in its interaction with CheZ,  thus affecting the ability of CheZ to bind and dephosphorylate it; or  (ii) the binding of CheY(N23D) to CheZ is stronger compared to  wild-type CheY, so that most of the CheZ present in the reaction would  be ```sequestered'''  leaving residual CheY(N23D), which would  be dephosphorylated only by spontaneous hydrolysis.	bind
16197	9	5580	7	10	NULL	NULL	NULL	CheY	GP	residual	dephosphorylated by		only	N23D		hydrolysis	Process	spontaneous			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_13_7357_s_57	8631757	(i) The  CheY(N23D) mutant protein is impaired in its interaction with CheZ,  thus affecting the ability of CheZ to bind and dephosphorylate it; or  (ii) the binding of CheY(N23D) to CheZ is stronger compared to  wild-type CheY, so that most of the CheZ present in the reaction would  be ```sequestered'''  leaving residual CheY(N23D), which would  be dephosphorylated only by spontaneous hydrolysis.	bind
16198	10	5580	7	10	NULL	NULL	NULL	statement 8	Process		leads to					statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_13_7357_s_57	8631757	(i) The  CheY(N23D) mutant protein is impaired in its interaction with CheZ,  thus affecting the ability of CheZ to bind and dephosphorylate it; or  (ii) the binding of CheY(N23D) to CheZ is stronger compared to  wild-type CheY, so that most of the CheZ present in the reaction would  be ```sequestered'''  leaving residual CheY(N23D), which would  be dephosphorylated only by spontaneous hydrolysis.	bind
16305	4	5580	7	10	NULL	NULL	NULL	statement 1	Process		affects					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_13_7357_s_57	8631757	(i) The  CheY(N23D) mutant protein is impaired in its interaction with CheZ,  thus affecting the ability of CheZ to bind and dephosphorylate it; or  (ii) the binding of CheY(N23D) to CheZ is stronger compared to  wild-type CheY, so that most of the CheZ present in the reaction would  be ```sequestered'''  leaving residual CheY(N23D), which would  be dephosphorylated only by spontaneous hydrolysis.	bind
20095	5	5580	7	10	NULL	NULL	NULL	CheY	GP	mutant	binds			N23D		CheZ	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_13_7357_s_57	8631757	(i) The  CheY(N23D) mutant protein is impaired in its interaction with CheZ,  thus affecting the ability of CheZ to bind and dephosphorylate it; or  (ii) the binding of CheY(N23D) to CheZ is stronger compared to  wild-type CheY, so that most of the CheZ present in the reaction would  be ```sequestered'''  leaving residual CheY(N23D), which would  be dephosphorylated only by spontaneous hydrolysis.	bind
20096	6	5580	7	10	NULL	NULL	NULL	CheY	GP	wild-type	binds					CheZ	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_13_7357_s_57	8631757	(i) The  CheY(N23D) mutant protein is impaired in its interaction with CheZ,  thus affecting the ability of CheZ to bind and dephosphorylate it; or  (ii) the binding of CheY(N23D) to CheZ is stronger compared to  wild-type CheY, so that most of the CheZ present in the reaction would  be ```sequestered'''  leaving residual CheY(N23D), which would  be dephosphorylated only by spontaneous hydrolysis.	bind
20097	7	5580	7	10	NULL	NULL	NULL	statement 5	Process		is stronger					statement 6	Process	compared to			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_13_7357_s_57	8631757	(i) The  CheY(N23D) mutant protein is impaired in its interaction with CheZ,  thus affecting the ability of CheZ to bind and dephosphorylate it; or  (ii) the binding of CheY(N23D) to CheZ is stronger compared to  wild-type CheY, so that most of the CheZ present in the reaction would  be ```sequestered'''  leaving residual CheY(N23D), which would  be dephosphorylated only by spontaneous hydrolysis.	bind
17236	1	5581	6	10	NULL	NULL	NULL				bind			CI		ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_9_2017_s_264	16628225	(i) The ATP binding modes between CI and CII differ ( Figure 1B) (  et al).	bind
17237	2	5581	6	10	NULL	NULL	NULL				bind			CII		ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_9_2017_s_264	16628225	(i) The ATP binding modes between CI and CII differ ( Figure 1B) (  et al).	bind
20036	3	5581	6	10	NULL	NULL	NULL	statement 1	Process	binding mode of	is different from					statement 2	Process	binding mode of 			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_9_2017_s_264	16628225	(i) The ATP binding modes between CI and CII differ ( Figure 1B) (  et al).	bind
16202	1	5581	7	10	NULL	NULL	NULL	ATP	Chemical		bind								CI		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_9_2017_s_264	16628225	(i) The ATP binding modes between CI and CII differ ( Figure 1B) (  et al).	bind
16203	2	5581	7	10	NULL	NULL	NULL	ATP	Chemical		bind								CII		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_9_2017_s_264	16628225	(i) The ATP binding modes between CI and CII differ ( Figure 1B) (  et al).	bind
16205	3	5581	7	10	NULL	NULL	NULL	statement 1	Process	binding mode of	differs with					statement 2	Process	binding mode of			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_9_2017_s_264	16628225	(i) The ATP binding modes between CI and CII differ ( Figure 1B) (  et al).	bind
17316	1	5582	6	10	NULL	NULL	NULL	ASF-1	GP		bind									as-1 element	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_3_775_s_171	11809891	(i) The binding affinity of ASF-1 and different TGA factors to the  as-1 element is highest if the spacing between the two palindromes is either 10 or 12 bp.	bind
17317	2	5582	6	10	NULL	NULL	NULL	TGA factors	GP		bind									as-1 element	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_3_775_s_171	11809891	(i) The binding affinity of ASF-1 and different TGA factors to the  as-1 element is highest if the spacing between the two palindromes is either 10 or 12 bp.	bind
16209	1	5582	7	10	NULL	NULL	NULL	ASF-1	GP		bind									as-1 element	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_3_775_s_171	11809891	(i) The binding affinity of ASF-1 and different TGA factors to the  as-1 element is highest if the spacing between the two palindromes is either 10 or 12 bp.	bind
16210	2	5582	7	10	NULL	NULL	NULL	TGA factors	GP		bind									as-1 element	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_3_775_s_171	11809891	(i) The binding affinity of ASF-1 and different TGA factors to the  as-1 element is highest if the spacing between the two palindromes is either 10 or 12 bp.	bind
17318	1	5583	6	10	NULL	NULL	NULL	alpha-Syn	GP		bind					phospholipids	Chemical	acidic			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_44_34328_s_135	10915790	(i) The binding of alpha-Syn with acidic phospholipids is dose-dependent; (ii) the extent of lipid binding depends rather on the availability of the phospholipids than on the size of lipid vesicles (SUVs  versus MLVs); (iii) alpha-Syn binding to phospholipid vesicles increases drastically when an acidic phospholipid is mixed with PE instead of PC; and (iv) alpha-Syn binding to acidic phospholipid (with PC or PE) vesicles is inversely proportional to the ionic strength.	bind
17320	2	5583	6	10	NULL	NULL	NULL	statement 1	Process		is dependent on					dose	QuantityOrMeasure				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_44_34328_s_135	10915790	(i) The binding of alpha-Syn with acidic phospholipids is dose-dependent; (ii) the extent of lipid binding depends rather on the availability of the phospholipids than on the size of lipid vesicles (SUVs  versus MLVs); (iii) alpha-Syn binding to phospholipid vesicles increases drastically when an acidic phospholipid is mixed with PE instead of PC; and (iv) alpha-Syn binding to acidic phospholipid (with PC or PE) vesicles is inversely proportional to the ionic strength.	bind
17323	3	5583	6	10	NULL	NULL	NULL	alpha-Syn	GP		bind					phospholipid vesicles	CellComponent	acidic			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_44_34328_s_135	10915790	(i) The binding of alpha-Syn with acidic phospholipids is dose-dependent; (ii) the extent of lipid binding depends rather on the availability of the phospholipids than on the size of lipid vesicles (SUVs  versus MLVs); (iii) alpha-Syn binding to phospholipid vesicles increases drastically when an acidic phospholipid is mixed with PE instead of PC; and (iv) alpha-Syn binding to acidic phospholipid (with PC or PE) vesicles is inversely proportional to the ionic strength.	bind
17727	4	5583	6	10	NULL	NULL	NULL	statement 3	Process		is inversely propotional to					ionic strength	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_44_34328_s_135	10915790	(i) The binding of alpha-Syn with acidic phospholipids is dose-dependent; (ii) the extent of lipid binding depends rather on the availability of the phospholipids than on the size of lipid vesicles (SUVs  versus MLVs); (iii) alpha-Syn binding to phospholipid vesicles increases drastically when an acidic phospholipid is mixed with PE instead of PC; and (iv) alpha-Syn binding to acidic phospholipid (with PC or PE) vesicles is inversely proportional to the ionic strength.	bind
20037	5	5583	6	10	NULL	NULL	NULL	alpha-Syn	GP		bind					phospholipid vesicles	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_44_34328_s_135	10915790	(i) The binding of alpha-Syn with acidic phospholipids is dose-dependent; (ii) the extent of lipid binding depends rather on the availability of the phospholipids than on the size of lipid vesicles (SUVs  versus MLVs); (iii) alpha-Syn binding to phospholipid vesicles increases drastically when an acidic phospholipid is mixed with PE instead of PC; and (iv) alpha-Syn binding to acidic phospholipid (with PC or PE) vesicles is inversely proportional to the ionic strength.	bind
16214	1	5583	7	10	NULL	NULL	NULL	alpha-Syn	GP		bind					 phospholipids	Chemical	acidic			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_44_34328_s_135	10915790	(i) The binding of alpha-Syn with acidic phospholipids is dose-dependent; (ii) the extent of lipid binding depends rather on the availability of the phospholipids than on the size of lipid vesicles (SUVs  versus MLVs); (iii) alpha-Syn binding to phospholipid vesicles increases drastically when an acidic phospholipid is mixed with PE instead of PC; and (iv) alpha-Syn binding to acidic phospholipid (with PC or PE) vesicles is inversely proportional to the ionic strength.	bind
16215	2	5583	7	10	NULL	NULL	NULL	statement 1	Process		is dependent on					dose	QuantityOrMeasure				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_44_34328_s_135	10915790	(i) The binding of alpha-Syn with acidic phospholipids is dose-dependent; (ii) the extent of lipid binding depends rather on the availability of the phospholipids than on the size of lipid vesicles (SUVs  versus MLVs); (iii) alpha-Syn binding to phospholipid vesicles increases drastically when an acidic phospholipid is mixed with PE instead of PC; and (iv) alpha-Syn binding to acidic phospholipid (with PC or PE) vesicles is inversely proportional to the ionic strength.	bind
16218	3	5583	7	10	NULL	NULL	NULL	alpha-Syn	GP		bind					phospholipid vesicles	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_44_34328_s_135	10915790	(i) The binding of alpha-Syn with acidic phospholipids is dose-dependent; (ii) the extent of lipid binding depends rather on the availability of the phospholipids than on the size of lipid vesicles (SUVs  versus MLVs); (iii) alpha-Syn binding to phospholipid vesicles increases drastically when an acidic phospholipid is mixed with PE instead of PC; and (iv) alpha-Syn binding to acidic phospholipid (with PC or PE) vesicles is inversely proportional to the ionic strength.	bind
16221	4	5583	7	10	NULL	NULL	NULL	alpha-Syn	GP		bind					phospholipid vesicles	CellComponent	acidic			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_44_34328_s_135	10915790	(i) The binding of alpha-Syn with acidic phospholipids is dose-dependent; (ii) the extent of lipid binding depends rather on the availability of the phospholipids than on the size of lipid vesicles (SUVs  versus MLVs); (iii) alpha-Syn binding to phospholipid vesicles increases drastically when an acidic phospholipid is mixed with PE instead of PC; and (iv) alpha-Syn binding to acidic phospholipid (with PC or PE) vesicles is inversely proportional to the ionic strength.	bind
16222	5	5583	7	10	NULL	NULL	NULL	statement 4	Process		is inversely proportional to					ionic strength	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_44_34328_s_135	10915790	(i) The binding of alpha-Syn with acidic phospholipids is dose-dependent; (ii) the extent of lipid binding depends rather on the availability of the phospholipids than on the size of lipid vesicles (SUVs  versus MLVs); (iii) alpha-Syn binding to phospholipid vesicles increases drastically when an acidic phospholipid is mixed with PE instead of PC; and (iv) alpha-Syn binding to acidic phospholipid (with PC or PE) vesicles is inversely proportional to the ionic strength.	bind
17327	1	5584	6	10	NULL	NULL	NULL	elongin C	GP		bind					VHL	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_33_30388_s_81	12048197	(i) The binding of Elongin C to VHL is stabilized by Elongin B both  in vitro and in cells ( 16,  35).	bind
17329	2	5584	6	10	NULL	NULL	NULL	Elongin B	GP		stabilizes					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_33_30388_s_81	12048197	(i) The binding of Elongin C to VHL is stabilized by Elongin B both  in vitro and in cells ( 16,  35).	bind
17330	4	5584	6	10	NULL	NULL	NULL	Elongin B	GP		stabilizes					statement 3	Process				NULL	in cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_33_30388_s_81	12048197	(i) The binding of Elongin C to VHL is stabilized by Elongin B both  in vitro and in cells ( 16,  35).	bind
17690	3	5584	6	10	NULL	NULL	NULL	elongin C	GP		bind					VHL	GP				NULL	in cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_33_30388_s_81	12048197	(i) The binding of Elongin C to VHL is stabilized by Elongin B both  in vitro and in cells ( 16,  35).	bind
16223	1	5584	7	10	NULL	NULL	NULL	Elongin C	GP		bind					VHL	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_33_30388_s_81	12048197	(i) The binding of Elongin C to VHL is stabilized by Elongin B both  in vitro and in cells ( 16,  35).	bind
16224	2	5584	7	10	NULL	NULL	NULL	Elongin C	GP		bind					VHL	GP				NULL	in cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_33_30388_s_81	12048197	(i) The binding of Elongin C to VHL is stabilized by Elongin B both  in vitro and in cells ( 16,  35).	bind
16225	3	5584	7	10	NULL	NULL	NULL	statement 1	Process		is stabilized by					Elongin B	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_33_30388_s_81	12048197	(i) The binding of Elongin C to VHL is stabilized by Elongin B both  in vitro and in cells ( 16,  35).	bind
16226	4	5584	7	10	NULL	NULL	NULL	statement 2	Process		is stabilized by					Elongin B	GP				NULL	in cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_33_30388_s_81	12048197	(i) The binding of Elongin C to VHL is stabilized by Elongin B both  in vitro and in cells ( 16,  35).	bind
17362	1	5585	6	10	NULL	NULL	NULL	Mg2+	Chemical		are located 			binding sites residues 457-464		central alpha2beta complex	GP	upstream of 	binding site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3583_s_269	10652354	(i) The binding sites of Mg2+ (residues 457-464) ( 40,  41), located upstream of the central alpha2beta complex binding site, form a part of the catalytic site of RNA polymerization.	bind
17363	2	5585	6	10	NULL	NULL	NULL	statement 1	Process		forms					RNA polymerization	Process		catalytic site 		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3583_s_269	10652354	(i) The binding sites of Mg2+ (residues 457-464) ( 40,  41), located upstream of the central alpha2beta complex binding site, form a part of the catalytic site of RNA polymerization.	bind
16227	1	5585	7	10	NULL	NULL	NULL	Mg2+	Chemical	 	is located			binding site residues 457-464		central alpha2beta complex	GP	upstream of 	 binding site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3583_s_269	10652354	(i) The binding sites of Mg2+ (residues 457-464) ( 40,  41), located upstream of the central alpha2beta complex binding site, form a part of the catalytic site of RNA polymerization.	bind
16228	2	5585	7	10	NULL	NULL	NULL	statement 1	Process		forms 					RNA polymerization	Process	part of 	catalytic site of		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3583_s_269	10652354	(i) The binding sites of Mg2+ (residues 457-464) ( 40,  41), located upstream of the central alpha2beta complex binding site, form a part of the catalytic site of RNA polymerization.	bind
17364	1	5587	6	10	NULL	NULL	NULL	NCAM	GP		bind			IgI domain		heparin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_15_10125_s_251	9092558	(i) The IgI domain bound heparin but did not bind other negatively charged carbohydrates such as carboxymethylated dextran (the surface of a CM5 sensor chip) and PSA. (ii) Other extracellular domains of NCAM (with the exception of the IgII domain) did not bind to heparin.	bind
17365	2	5587	6	10	NULL	NULL	NULL	NCAM	GP		does not bind			IgI domain		carboxymethylated dextran	Chemical	negatively charged			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_15_10125_s_251	9092558	(i) The IgI domain bound heparin but did not bind other negatively charged carbohydrates such as carboxymethylated dextran (the surface of a CM5 sensor chip) and PSA. (ii) Other extracellular domains of NCAM (with the exception of the IgII domain) did not bind to heparin.	bind
17366	3	5587	6	10	NULL	NULL	NULL	NCAM	GP		does not bind			IgI domain		PSA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_15_10125_s_251	9092558	(i) The IgI domain bound heparin but did not bind other negatively charged carbohydrates such as carboxymethylated dextran (the surface of a CM5 sensor chip) and PSA. (ii) Other extracellular domains of NCAM (with the exception of the IgII domain) did not bind to heparin.	bind
17367	4	5587	6	10	NULL	NULL	NULL	NCAM	GP		bind			IgII domain		heparin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_15_10125_s_251	9092558	(i) The IgI domain bound heparin but did not bind other negatively charged carbohydrates such as carboxymethylated dextran (the surface of a CM5 sensor chip) and PSA. (ii) Other extracellular domains of NCAM (with the exception of the IgII domain) did not bind to heparin.	bind
17368	5	5587	6	10	NULL	NULL	NULL	NCAM	GP		does not bind			extracellular domain		heparin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_15_10125_s_251	9092558	(i) The IgI domain bound heparin but did not bind other negatively charged carbohydrates such as carboxymethylated dextran (the surface of a CM5 sensor chip) and PSA. (ii) Other extracellular domains of NCAM (with the exception of the IgII domain) did not bind to heparin.	bind
16229	1	5587	7	10	NULL	NULL	NULL	NCAM	GP		bind			 IgI 		heparin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_15_10125_s_251	9092558	(i) The IgI domain bound heparin but did not bind other negatively charged carbohydrates such as carboxymethylated dextran (the surface of a CM5 sensor chip) and PSA. (ii) Other extracellular domains of NCAM (with the exception of the IgII domain) did not bind to heparin.	bind
16230	2	5587	7	10	NULL	NULL	NULL	NCAM	GP		does not bind			IgI		carboxymethylated dextran	Chemical	negatively charged			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_15_10125_s_251	9092558	(i) The IgI domain bound heparin but did not bind other negatively charged carbohydrates such as carboxymethylated dextran (the surface of a CM5 sensor chip) and PSA. (ii) Other extracellular domains of NCAM (with the exception of the IgII domain) did not bind to heparin.	bind
16231	3	5587	7	10	NULL	NULL	NULL	NCAM	GP		does not bind			IgI		PSA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_15_10125_s_251	9092558	(i) The IgI domain bound heparin but did not bind other negatively charged carbohydrates such as carboxymethylated dextran (the surface of a CM5 sensor chip) and PSA. (ii) Other extracellular domains of NCAM (with the exception of the IgII domain) did not bind to heparin.	bind
16232	4	5587	7	10	NULL	NULL	NULL	NCAM	GP	 	does not bind			extracellular domain		heparin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_15_10125_s_251	9092558	(i) The IgI domain bound heparin but did not bind other negatively charged carbohydrates such as carboxymethylated dextran (the surface of a CM5 sensor chip) and PSA. (ii) Other extracellular domains of NCAM (with the exception of the IgII domain) did not bind to heparin.	bind
16233	5	5587	7	10	NULL	NULL	NULL	NCAM	GP		bind			IgII		heparin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_15_10125_s_251	9092558	(i) The IgI domain bound heparin but did not bind other negatively charged carbohydrates such as carboxymethylated dextran (the surface of a CM5 sensor chip) and PSA. (ii) Other extracellular domains of NCAM (with the exception of the IgII domain) did not bind to heparin.	bind
17369	1	5588	6	10	NULL	NULL	NULL	ctMycBR Max heterodimer	GP		does not bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_48_28797_s_230	7499403	(i) The presence of Max does  not confer DNA binding activity to the  ctMycBR  Max heterodimer.	bind
20038	2	5588	6	10	NULL	NULL	NULL	Max	GP	presence of	does not confer					ctMycBR Max heterodimer	GP	DNA binding activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_48_28797_s_230	7499403	(i) The presence of Max does  not confer DNA binding activity to the  ctMycBR  Max heterodimer.	bind
16236	1	5588	7	10	NULL	NULL	NULL	ctMycBR Max heterodimer 	GP		does not bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_48_28797_s_230	7499403	(i) The presence of Max does  not confer DNA binding activity to the  ctMycBR  Max heterodimer.	bind
16238	2	5588	7	10	NULL	NULL	NULL	Max	GP	presence of 	does not confer					ctMycBR Max heterodimer	GP	DNA binding activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_48_28797_s_230	7499403	(i) The presence of Max does  not confer DNA binding activity to the  ctMycBR  Max heterodimer.	bind
17370	1	5589	6	10	NULL	NULL	NULL	Zw5 protein	GP		bind									scs	NULL		NULL	NULL	NULL	NULL	gw70_embo_24_2_358_s_195	15650749	(I) The proteins Zw5 and BEAF, which  bind to the insulator elements  scs and  scs'', interact with each other  in vitro and their binding sites are located in close proximity to each other  in vivo (  et al).	bind
17371	2	5589	6	10	NULL	NULL	NULL	BEAF protein	GP		bind									scs''	NULL		NULL	NULL	NULL	NULL	gw70_embo_24_2_358_s_195	15650749	(I) The proteins Zw5 and BEAF, which  bind to the insulator elements  scs and  scs'', interact with each other  in vitro and their binding sites are located in close proximity to each other  in vivo (  et al).	bind
17374	3	5589	6	10	NULL	NULL	NULL	Zw5	GP		interact with					BEAF	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_embo_24_2_358_s_195	15650749	(I) The proteins Zw5 and BEAF, which  bind to the insulator elements  scs and  scs'', interact with each other  in vitro and their binding sites are located in close proximity to each other  in vivo (  et al).	bind
20039	4	5589	6	NULL	NULL	0	NULL		NULL		is in close proximity to	NULL			scs		NULL			scs''	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_embo_24_2_358_s_195	15650749	(I) The proteins Zw5 and BEAF, which  bind to the insulator elements  scs and  scs'', interact with each other  in vitro and their binding sites are located in close proximity to each other  in vivo (  et al).	bind
53188	5	5589	6	10	NULL	NULL	NULL	scs	GP		is a type of					insulator element	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_2_358_s_195	15650749	(I) The proteins Zw5 and BEAF, which  bind to the insulator elements  scs and  scs'', interact with each other  in vitro and their binding sites are located in close proximity to each other  in vivo (  et al).	bind
53189	6	5589	6	10	NULL	NULL	NULL	scs''	GP		is a type of					insulator element	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_2_358_s_195	15650749	(I) The proteins Zw5 and BEAF, which  bind to the insulator elements  scs and  scs'', interact with each other  in vitro and their binding sites are located in close proximity to each other  in vivo (  et al).	bind
16239	1	5589	7	10	NULL	NULL	NULL	Zw5 protein	GP		bind									scs	NULL		NULL	NULL	NULL	NULL	gw70_embo_24_2_358_s_195	15650749	(I) The proteins Zw5 and BEAF, which  bind to the insulator elements  scs and  scs'', interact with each other  in vitro and their binding sites are located in close proximity to each other  in vivo (  et al).	bind
16240	2	5589	7	10	NULL	NULL	NULL	BEAF protein	GP		bind									scs''	NULL		NULL	NULL	NULL	NULL	gw70_embo_24_2_358_s_195	15650749	(I) The proteins Zw5 and BEAF, which  bind to the insulator elements  scs and  scs'', interact with each other  in vitro and their binding sites are located in close proximity to each other  in vivo (  et al).	bind
16243	5	5589	7	10	NULL	NULL	NULL	Zw5	GP		interacts with					BEAF	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_embo_24_2_358_s_195	15650749	(I) The proteins Zw5 and BEAF, which  bind to the insulator elements  scs and  scs'', interact with each other  in vitro and their binding sites are located in close proximity to each other  in vivo (  et al).	bind
16244	6	5589	7	NULL	NULL	0	NULL		NULL		is in close proximity to	NULL			scs		NULL			scs''	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_embo_24_2_358_s_195	15650749	(I) The proteins Zw5 and BEAF, which  bind to the insulator elements  scs and  scs'', interact with each other  in vitro and their binding sites are located in close proximity to each other  in vivo (  et al).	bind
53190	3	5589	7	10	NULL	NULL	NULL	scs	GP		is a type of					insulator element	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_2_358_s_195	15650749	(I) The proteins Zw5 and BEAF, which  bind to the insulator elements  scs and  scs'', interact with each other  in vitro and their binding sites are located in close proximity to each other  in vivo (  et al).	bind
53191	4	5589	7	10	NULL	NULL	NULL	scs''	GP		is a type of					insulator element	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_2_358_s_195	15650749	(I) The proteins Zw5 and BEAF, which  bind to the insulator elements  scs and  scs'', interact with each other  in vitro and their binding sites are located in close proximity to each other  in vivo (  et al).	bind
17375	1	5590	6	10	NULL	NULL	NULL	NADPH	Chemical		bind		tightly			EH2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_48_37317_s_243	10969088	(i) The redox potentials of  EH2/ EH4,  325 mV for the  E. coli and human enzymes, ( 24) and of NADP+/NADPH,  309 mV at pH 6.9 and 25  degrees C ( 25), together with the high NADPH concentration determine the effective redox potential of the system; (ii) the binding of NADPH to  EH2 is very tight, and we assume that it is tighter than the binding to  EH4; this causes the redox potential of the system to be shifted to even more negative values ( 26).	bind
17376	2	5590	6	10	NULL	NULL	NULL	NADPH	Chemical		bind					EH4	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_48_37317_s_243	10969088	(i) The redox potentials of  EH2/ EH4,  325 mV for the  E. coli and human enzymes, ( 24) and of NADP+/NADPH,  309 mV at pH 6.9 and 25  degrees C ( 25), together with the high NADPH concentration determine the effective redox potential of the system; (ii) the binding of NADPH to  EH2 is very tight, and we assume that it is tighter than the binding to  EH4; this causes the redox potential of the system to be shifted to even more negative values ( 26).	bind
17377	3	5590	6	10	NULL	NULL	NULL	statement 1	Process		is stronger than		probably			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_48_37317_s_243	10969088	(i) The redox potentials of  EH2/ EH4,  325 mV for the  E. coli and human enzymes, ( 24) and of NADP+/NADPH,  309 mV at pH 6.9 and 25  degrees C ( 25), together with the high NADPH concentration determine the effective redox potential of the system; (ii) the binding of NADPH to  EH2 is very tight, and we assume that it is tighter than the binding to  EH4; this causes the redox potential of the system to be shifted to even more negative values ( 26).	bind
20040	4	5590	6	10	NULL	NULL	NULL	statement 1	Process		cause					redox potential	QuantityOrMeasure	negative value of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_48_37317_s_243	10969088	(i) The redox potentials of  EH2/ EH4,  325 mV for the  E. coli and human enzymes, ( 24) and of NADP+/NADPH,  309 mV at pH 6.9 and 25  degrees C ( 25), together with the high NADPH concentration determine the effective redox potential of the system; (ii) the binding of NADPH to  EH2 is very tight, and we assume that it is tighter than the binding to  EH4; this causes the redox potential of the system to be shifted to even more negative values ( 26).	bind
16245	1	5590	7	10	NULL	NULL	NULL	NADPH	Chemical		bind		tightly			EH2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_48_37317_s_243	10969088	(i) The redox potentials of  EH2/ EH4,  325 mV for the  E. coli and human enzymes, ( 24) and of NADP+/NADPH,  309 mV at pH 6.9 and 25  degrees C ( 25), together with the high NADPH concentration determine the effective redox potential of the system; (ii) the binding of NADPH to  EH2 is very tight, and we assume that it is tighter than the binding to  EH4; this causes the redox potential of the system to be shifted to even more negative values ( 26).	bind
16246	2	5590	7	10	NULL	NULL	NULL	NADPH	Chemical		bind					EH4	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_48_37317_s_243	10969088	(i) The redox potentials of  EH2/ EH4,  325 mV for the  E. coli and human enzymes, ( 24) and of NADP+/NADPH,  309 mV at pH 6.9 and 25  degrees C ( 25), together with the high NADPH concentration determine the effective redox potential of the system; (ii) the binding of NADPH to  EH2 is very tight, and we assume that it is tighter than the binding to  EH4; this causes the redox potential of the system to be shifted to even more negative values ( 26).	bind
16247	3	5590	7	10	NULL	NULL	NULL	statement 1	Process		is tighter than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_48_37317_s_243	10969088	(i) The redox potentials of  EH2/ EH4,  325 mV for the  E. coli and human enzymes, ( 24) and of NADP+/NADPH,  309 mV at pH 6.9 and 25  degrees C ( 25), together with the high NADPH concentration determine the effective redox potential of the system; (ii) the binding of NADPH to  EH2 is very tight, and we assume that it is tighter than the binding to  EH4; this causes the redox potential of the system to be shifted to even more negative values ( 26).	bind
16248	4	5590	7	10	NULL	NULL	NULL	statement 1	Process		cause					 redox potential	QuantityOrMeasure	negative value of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_48_37317_s_243	10969088	(i) The redox potentials of  EH2/ EH4,  325 mV for the  E. coli and human enzymes, ( 24) and of NADP+/NADPH,  309 mV at pH 6.9 and 25  degrees C ( 25), together with the high NADPH concentration determine the effective redox potential of the system; (ii) the binding of NADPH to  EH2 is very tight, and we assume that it is tighter than the binding to  EH4; this causes the redox potential of the system to be shifted to even more negative values ( 26).	bind
17678	1	5591	6	10	NULL	NULL	NULL	RelA	GP		forms heteromer with					C/EBP	GP				NULL	LPS-induced rabbit liver	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7365_s_267	7706280	(i) There is  in vivo  evidence of  RelA C/EBP heteromer formation at the SAA promoter in the  LPS-induced rabbit liver; (ii) RelA and C/EBP-   cooperatively  transactivate the expression of SAA gene; (iii) the heteromeric complex  of NF-kappaB and C/EBP has a higher transactivation potential in  activating SAA expression than their homomeric counterparts; (iv) the  heteromeric complex of NF-kappaB and C/EBP can bind to both NF-kappaB  and C/EBP binding elements; (v) the NF-kappaB C/EBP heteromer  interacts with the NF-kappaB element with a much higher affinity than  that with the C/EBP element of SAA promoter.	bind
17679	2	5591	6	10	NULL	NULL	NULL	RelA	GP		transactivate					SAA gene	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7365_s_267	7706280	(i) There is  in vivo  evidence of  RelA C/EBP heteromer formation at the SAA promoter in the  LPS-induced rabbit liver; (ii) RelA and C/EBP-   cooperatively  transactivate the expression of SAA gene; (iii) the heteromeric complex  of NF-kappaB and C/EBP has a higher transactivation potential in  activating SAA expression than their homomeric counterparts; (iv) the  heteromeric complex of NF-kappaB and C/EBP can bind to both NF-kappaB  and C/EBP binding elements; (v) the NF-kappaB C/EBP heteromer  interacts with the NF-kappaB element with a much higher affinity than  that with the C/EBP element of SAA promoter.	bind
17680	3	5591	6	10	NULL	NULL	NULL	C/EBP	GP		transactivate					SAA gene	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7365_s_267	7706280	(i) There is  in vivo  evidence of  RelA C/EBP heteromer formation at the SAA promoter in the  LPS-induced rabbit liver; (ii) RelA and C/EBP-   cooperatively  transactivate the expression of SAA gene; (iii) the heteromeric complex  of NF-kappaB and C/EBP has a higher transactivation potential in  activating SAA expression than their homomeric counterparts; (iv) the  heteromeric complex of NF-kappaB and C/EBP can bind to both NF-kappaB  and C/EBP binding elements; (v) the NF-kappaB C/EBP heteromer  interacts with the NF-kappaB element with a much higher affinity than  that with the C/EBP element of SAA promoter.	bind
17681	4	5591	6	10	NULL	NULL	NULL	statement 2	Process		acts in cooperation with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7365_s_267	7706280	(i) There is  in vivo  evidence of  RelA C/EBP heteromer formation at the SAA promoter in the  LPS-induced rabbit liver; (ii) RelA and C/EBP-   cooperatively  transactivate the expression of SAA gene; (iii) the heteromeric complex  of NF-kappaB and C/EBP has a higher transactivation potential in  activating SAA expression than their homomeric counterparts; (iv) the  heteromeric complex of NF-kappaB and C/EBP can bind to both NF-kappaB  and C/EBP binding elements; (v) the NF-kappaB C/EBP heteromer  interacts with the NF-kappaB element with a much higher affinity than  that with the C/EBP element of SAA promoter.	bind
17682	5	5591	6	10	NULL	NULL	NULL	NF-kappaB	GP		forms a heteromeric complex with					C/EBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7365_s_267	7706280	(i) There is  in vivo  evidence of  RelA C/EBP heteromer formation at the SAA promoter in the  LPS-induced rabbit liver; (ii) RelA and C/EBP-   cooperatively  transactivate the expression of SAA gene; (iii) the heteromeric complex  of NF-kappaB and C/EBP has a higher transactivation potential in  activating SAA expression than their homomeric counterparts; (iv) the  heteromeric complex of NF-kappaB and C/EBP can bind to both NF-kappaB  and C/EBP binding elements; (v) the NF-kappaB C/EBP heteromer  interacts with the NF-kappaB element with a much higher affinity than  that with the C/EBP element of SAA promoter.	bind
17683	6	5591	6	10	NULL	NULL	NULL	statement 5	Process		bind					SAA	GP			NF-kappaB-binding element of promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7365_s_267	7706280	(i) There is  in vivo  evidence of  RelA C/EBP heteromer formation at the SAA promoter in the  LPS-induced rabbit liver; (ii) RelA and C/EBP-   cooperatively  transactivate the expression of SAA gene; (iii) the heteromeric complex  of NF-kappaB and C/EBP has a higher transactivation potential in  activating SAA expression than their homomeric counterparts; (iv) the  heteromeric complex of NF-kappaB and C/EBP can bind to both NF-kappaB  and C/EBP binding elements; (v) the NF-kappaB C/EBP heteromer  interacts with the NF-kappaB element with a much higher affinity than  that with the C/EBP element of SAA promoter.	bind
17684	7	5591	6	10	NULL	NULL	NULL	statement 5	Process		bind					SAA	GP			C/EBP binding element of promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7365_s_267	7706280	(i) There is  in vivo  evidence of  RelA C/EBP heteromer formation at the SAA promoter in the  LPS-induced rabbit liver; (ii) RelA and C/EBP-   cooperatively  transactivate the expression of SAA gene; (iii) the heteromeric complex  of NF-kappaB and C/EBP has a higher transactivation potential in  activating SAA expression than their homomeric counterparts; (iv) the  heteromeric complex of NF-kappaB and C/EBP can bind to both NF-kappaB  and C/EBP binding elements; (v) the NF-kappaB C/EBP heteromer  interacts with the NF-kappaB element with a much higher affinity than  that with the C/EBP element of SAA promoter.	bind
17731	8	5591	6	10	NULL	NULL	NULL	statement 1	Process		bind					SAA	GP			promoter	NULL	LPS-induced rabbit liver	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7365_s_267	7706280	(i) There is  in vivo  evidence of  RelA C/EBP heteromer formation at the SAA promoter in the  LPS-induced rabbit liver; (ii) RelA and C/EBP-   cooperatively  transactivate the expression of SAA gene; (iii) the heteromeric complex  of NF-kappaB and C/EBP has a higher transactivation potential in  activating SAA expression than their homomeric counterparts; (iv) the  heteromeric complex of NF-kappaB and C/EBP can bind to both NF-kappaB  and C/EBP binding elements; (v) the NF-kappaB C/EBP heteromer  interacts with the NF-kappaB element with a much higher affinity than  that with the C/EBP element of SAA promoter.	bind
17732	9	5591	6	10	NULL	NULL	NULL	statement 6	Process		has much higher affinity than					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7365_s_267	7706280	(i) There is  in vivo  evidence of  RelA C/EBP heteromer formation at the SAA promoter in the  LPS-induced rabbit liver; (ii) RelA and C/EBP-   cooperatively  transactivate the expression of SAA gene; (iii) the heteromeric complex  of NF-kappaB and C/EBP has a higher transactivation potential in  activating SAA expression than their homomeric counterparts; (iv) the  heteromeric complex of NF-kappaB and C/EBP can bind to both NF-kappaB  and C/EBP binding elements; (v) the NF-kappaB C/EBP heteromer  interacts with the NF-kappaB element with a much higher affinity than  that with the C/EBP element of SAA promoter.	bind
20301	10	5591	6	10	NULL	NULL	NULL	NF-kappaB C/EBP heteromeric complex	GP	transactivation potential of	is higher than					homomeric counterparts	GP	transactivation potential of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7365_s_267	7706280	(i) There is  in vivo  evidence of  RelA C/EBP heteromer formation at the SAA promoter in the  LPS-induced rabbit liver; (ii) RelA and C/EBP-   cooperatively  transactivate the expression of SAA gene; (iii) the heteromeric complex  of NF-kappaB and C/EBP has a higher transactivation potential in  activating SAA expression than their homomeric counterparts; (iv) the  heteromeric complex of NF-kappaB and C/EBP can bind to both NF-kappaB  and C/EBP binding elements; (v) the NF-kappaB C/EBP heteromer  interacts with the NF-kappaB element with a much higher affinity than  that with the C/EBP element of SAA promoter.	bind
53193	11	5591	6	10	NULL	NULL	NULL	statement 5	Process		activates					SAA	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7365_s_267	7706280	(i) There is  in vivo  evidence of  RelA C/EBP heteromer formation at the SAA promoter in the  LPS-induced rabbit liver; (ii) RelA and C/EBP-   cooperatively  transactivate the expression of SAA gene; (iii) the heteromeric complex  of NF-kappaB and C/EBP has a higher transactivation potential in  activating SAA expression than their homomeric counterparts; (iv) the  heteromeric complex of NF-kappaB and C/EBP can bind to both NF-kappaB  and C/EBP binding elements; (v) the NF-kappaB C/EBP heteromer  interacts with the NF-kappaB element with a much higher affinity than  that with the C/EBP element of SAA promoter.	bind
16249	1	5591	7	10	NULL	NULL	NULL	RelA	GP		transactivate					SAA 	GP	 expression of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7365_s_267	7706280	(i) There is  in vivo  evidence of  RelA C/EBP heteromer formation at the SAA promoter in the  LPS-induced rabbit liver; (ii) RelA and C/EBP-   cooperatively  transactivate the expression of SAA gene; (iii) the heteromeric complex  of NF-kappaB and C/EBP has a higher transactivation potential in  activating SAA expression than their homomeric counterparts; (iv) the  heteromeric complex of NF-kappaB and C/EBP can bind to both NF-kappaB  and C/EBP binding elements; (v) the NF-kappaB C/EBP heteromer  interacts with the NF-kappaB element with a much higher affinity than  that with the C/EBP element of SAA promoter.	bind
16250	2	5591	7	10	NULL	NULL	NULL	C/EBP	GP		transactivate					SAA	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7365_s_267	7706280	(i) There is  in vivo  evidence of  RelA C/EBP heteromer formation at the SAA promoter in the  LPS-induced rabbit liver; (ii) RelA and C/EBP-   cooperatively  transactivate the expression of SAA gene; (iii) the heteromeric complex  of NF-kappaB and C/EBP has a higher transactivation potential in  activating SAA expression than their homomeric counterparts; (iv) the  heteromeric complex of NF-kappaB and C/EBP can bind to both NF-kappaB  and C/EBP binding elements; (v) the NF-kappaB C/EBP heteromer  interacts with the NF-kappaB element with a much higher affinity than  that with the C/EBP element of SAA promoter.	bind
16251	3	5591	7	10	NULL	NULL	NULL	statement 1	Process		occurs in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7365_s_267	7706280	(i) There is  in vivo  evidence of  RelA C/EBP heteromer formation at the SAA promoter in the  LPS-induced rabbit liver; (ii) RelA and C/EBP-   cooperatively  transactivate the expression of SAA gene; (iii) the heteromeric complex  of NF-kappaB and C/EBP has a higher transactivation potential in  activating SAA expression than their homomeric counterparts; (iv) the  heteromeric complex of NF-kappaB and C/EBP can bind to both NF-kappaB  and C/EBP binding elements; (v) the NF-kappaB C/EBP heteromer  interacts with the NF-kappaB element with a much higher affinity than  that with the C/EBP element of SAA promoter.	bind
16252	4	5591	7	10	NULL	NULL	NULL	NF-kappaB	GP		forms heteromeric complex with					C/EBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7365_s_267	7706280	(i) There is  in vivo  evidence of  RelA C/EBP heteromer formation at the SAA promoter in the  LPS-induced rabbit liver; (ii) RelA and C/EBP-   cooperatively  transactivate the expression of SAA gene; (iii) the heteromeric complex  of NF-kappaB and C/EBP has a higher transactivation potential in  activating SAA expression than their homomeric counterparts; (iv) the  heteromeric complex of NF-kappaB and C/EBP can bind to both NF-kappaB  and C/EBP binding elements; (v) the NF-kappaB C/EBP heteromer  interacts with the NF-kappaB element with a much higher affinity than  that with the C/EBP element of SAA promoter.	bind
16253	5	5591	7	10	NULL	NULL	NULL	statement 4	Process		activates					SAA	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7365_s_267	7706280	(i) There is  in vivo  evidence of  RelA C/EBP heteromer formation at the SAA promoter in the  LPS-induced rabbit liver; (ii) RelA and C/EBP-   cooperatively  transactivate the expression of SAA gene; (iii) the heteromeric complex  of NF-kappaB and C/EBP has a higher transactivation potential in  activating SAA expression than their homomeric counterparts; (iv) the  heteromeric complex of NF-kappaB and C/EBP can bind to both NF-kappaB  and C/EBP binding elements; (v) the NF-kappaB C/EBP heteromer  interacts with the NF-kappaB element with a much higher affinity than  that with the C/EBP element of SAA promoter.	bind
16254	6	5591	7	10	NULL	NULL	NULL	NF-kappaB C/EBP heteromeric complex	GP	transactivation potential of	is high than					homomeric counterparts	GP	transactivation potential of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7365_s_267	7706280	(i) There is  in vivo  evidence of  RelA C/EBP heteromer formation at the SAA promoter in the  LPS-induced rabbit liver; (ii) RelA and C/EBP-   cooperatively  transactivate the expression of SAA gene; (iii) the heteromeric complex  of NF-kappaB and C/EBP has a higher transactivation potential in  activating SAA expression than their homomeric counterparts; (iv) the  heteromeric complex of NF-kappaB and C/EBP can bind to both NF-kappaB  and C/EBP binding elements; (v) the NF-kappaB C/EBP heteromer  interacts with the NF-kappaB element with a much higher affinity than  that with the C/EBP element of SAA promoter.	bind
16255	7	5591	7	10	NULL	NULL	NULL	statement 4	Process		bind					SAA	GP			NF-kappaB binding element	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7365_s_267	7706280	(i) There is  in vivo  evidence of  RelA C/EBP heteromer formation at the SAA promoter in the  LPS-induced rabbit liver; (ii) RelA and C/EBP-   cooperatively  transactivate the expression of SAA gene; (iii) the heteromeric complex  of NF-kappaB and C/EBP has a higher transactivation potential in  activating SAA expression than their homomeric counterparts; (iv) the  heteromeric complex of NF-kappaB and C/EBP can bind to both NF-kappaB  and C/EBP binding elements; (v) the NF-kappaB C/EBP heteromer  interacts with the NF-kappaB element with a much higher affinity than  that with the C/EBP element of SAA promoter.	bind
16256	8	5591	7	10	NULL	NULL	NULL	statement 4	Process		bind					SAA	GP			C/EBP binding element	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7365_s_267	7706280	(i) There is  in vivo  evidence of  RelA C/EBP heteromer formation at the SAA promoter in the  LPS-induced rabbit liver; (ii) RelA and C/EBP-   cooperatively  transactivate the expression of SAA gene; (iii) the heteromeric complex  of NF-kappaB and C/EBP has a higher transactivation potential in  activating SAA expression than their homomeric counterparts; (iv) the  heteromeric complex of NF-kappaB and C/EBP can bind to both NF-kappaB  and C/EBP binding elements; (v) the NF-kappaB C/EBP heteromer  interacts with the NF-kappaB element with a much higher affinity than  that with the C/EBP element of SAA promoter.	bind
16257	9	5591	7	10	NULL	NULL	NULL	statement 7	Process		has higher affinity than					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7365_s_267	7706280	(i) There is  in vivo  evidence of  RelA C/EBP heteromer formation at the SAA promoter in the  LPS-induced rabbit liver; (ii) RelA and C/EBP-   cooperatively  transactivate the expression of SAA gene; (iii) the heteromeric complex  of NF-kappaB and C/EBP has a higher transactivation potential in  activating SAA expression than their homomeric counterparts; (iv) the  heteromeric complex of NF-kappaB and C/EBP can bind to both NF-kappaB  and C/EBP binding elements; (v) the NF-kappaB C/EBP heteromer  interacts with the NF-kappaB element with a much higher affinity than  that with the C/EBP element of SAA promoter.	bind
20094	10	5591	7	10	NULL	NULL	NULL	RelA	GP		forms heteromer with					C/EBP	GP				NULL	LPS-induced rabbit liver	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7365_s_267	7706280	(i) There is  in vivo  evidence of  RelA C/EBP heteromer formation at the SAA promoter in the  LPS-induced rabbit liver; (ii) RelA and C/EBP-   cooperatively  transactivate the expression of SAA gene; (iii) the heteromeric complex  of NF-kappaB and C/EBP has a higher transactivation potential in  activating SAA expression than their homomeric counterparts; (iv) the  heteromeric complex of NF-kappaB and C/EBP can bind to both NF-kappaB  and C/EBP binding elements; (v) the NF-kappaB C/EBP heteromer  interacts with the NF-kappaB element with a much higher affinity than  that with the C/EBP element of SAA promoter.	bind
53192	11	5591	7	10	NULL	NULL	NULL	statement 8	Process		bind					SAA	GP			promoter	NULL	LPS-induced rabbit liver	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7365_s_267	7706280	(i) There is  in vivo  evidence of  RelA C/EBP heteromer formation at the SAA promoter in the  LPS-induced rabbit liver; (ii) RelA and C/EBP-   cooperatively  transactivate the expression of SAA gene; (iii) the heteromeric complex  of NF-kappaB and C/EBP has a higher transactivation potential in  activating SAA expression than their homomeric counterparts; (iv) the  heteromeric complex of NF-kappaB and C/EBP can bind to both NF-kappaB  and C/EBP binding elements; (v) the NF-kappaB C/EBP heteromer  interacts with the NF-kappaB element with a much higher affinity than  that with the C/EBP element of SAA promoter.	bind
17378	1	5593	6	10	NULL	NULL	NULL	Hsc70	GP		bind					HRI	GP	transformed			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_5861_s_356	10454533	(i) Under conditions of heme deficiency, the binding of Hsc70 to transformed HRI may directly suppress its autokinase activity, preventing the hyperphosphorylation of transformed HRI (Fig.  10B,  1).	bind
17380	2	5593	6	10	NULL	NULL	NULL	statement 1	Process		suppress		may directly			Hsc70	GP	autokinase activity of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_5861_s_356	10454533	(i) Under conditions of heme deficiency, the binding of Hsc70 to transformed HRI may directly suppress its autokinase activity, preventing the hyperphosphorylation of transformed HRI (Fig.  10B,  1).	bind
17382	3	5593	6	10	NULL	NULL	NULL	statement 2	Process		prevents					HRI	GP	hyperphosphorylation transformed			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_5861_s_356	10454533	(i) Under conditions of heme deficiency, the binding of Hsc70 to transformed HRI may directly suppress its autokinase activity, preventing the hyperphosphorylation of transformed HRI (Fig.  10B,  1).	bind
17384	4	5593	6	10	NULL	NULL	NULL	statement 2	Process		occurs under					heme	Chemical	deficiency of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_5861_s_356	10454533	(i) Under conditions of heme deficiency, the binding of Hsc70 to transformed HRI may directly suppress its autokinase activity, preventing the hyperphosphorylation of transformed HRI (Fig.  10B,  1).	bind
16258	1	5593	7	10	NULL	NULL	NULL	Hsc70	GP		bind					HRI	GP	transformed			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_5861_s_356	10454533	(i) Under conditions of heme deficiency, the binding of Hsc70 to transformed HRI may directly suppress its autokinase activity, preventing the hyperphosphorylation of transformed HRI (Fig.  10B,  1).	bind
16259	2	5593	7	10	NULL	NULL	NULL	statement 1	Process		occurs under					heme	Chemical	deficiency of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_5861_s_356	10454533	(i) Under conditions of heme deficiency, the binding of Hsc70 to transformed HRI may directly suppress its autokinase activity, preventing the hyperphosphorylation of transformed HRI (Fig.  10B,  1).	bind
16260	3	5593	7	10	NULL	NULL	NULL	statement 1	Process		suppress		may directly			Hsc70	GP	autokinase activity of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_5861_s_356	10454533	(i) Under conditions of heme deficiency, the binding of Hsc70 to transformed HRI may directly suppress its autokinase activity, preventing the hyperphosphorylation of transformed HRI (Fig.  10B,  1).	bind
16261	4	5593	7	10	NULL	NULL	NULL	statement 1	Process		prevents					HRI	GP	hyperphosphorylation of transformed			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_5861_s_356	10454533	(i) Under conditions of heme deficiency, the binding of Hsc70 to transformed HRI may directly suppress its autokinase activity, preventing the hyperphosphorylation of transformed HRI (Fig.  10B,  1).	bind
17386	1	5594	6	10	NULL	NULL	NULL	basal AP-2	GP	binding of	does not change with					ischemia	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_45_16345_s_136	16258061	(I) versus nonischemic (N) limbs, no binding of YB-1, and no  change in basal AP-2 binding with ischemia.	bind
16446	1	5594	7	10	NULL	NULL	NULL	basal AP-2	GP	 binding of	does not change with					ischemia	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_45_16345_s_136	16258061	(I) versus nonischemic (N) limbs, no binding of YB-1, and no  change in basal AP-2 binding with ischemia.	bind
17393	1	5595	6	10	NULL	NULL	NULL	homodimeric SRF	GP		bind									SRE motif	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_17_12941_s_104	10777594	(I) was formed by a homodimeric SRF bound to the SRE motif.	bind
16312	1	5595	7	10	NULL	NULL	NULL	 homodimeric SRF	GP		bind									SRE motif	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_17_12941_s_104	10777594	(I) was formed by a homodimeric SRF bound to the SRE motif.	bind
17396	1	5596	6	10	NULL	NULL	NULL	low molecular weight protein cDNA	NucleicAcid		bind		specifically			hYAP	GP		WW domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_24_14733_s_133	7782338	(i) We have recently  identified and cloned two cDNAs for low molecular weight proteins that  bind specifically to the WW domain of hYAP.	bind
16313	1	5596	7	10	NULL	NULL	NULL	low molecular weight protein cDNA	NucleicAcid		bind		specifically			hYAP	GP		 WW domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_24_14733_s_133	7782338	(i) We have recently  identified and cloned two cDNAs for low molecular weight proteins that  bind specifically to the WW domain of hYAP.	bind
17400	1	5597	6	NULL	NULL	0	NULL		NULL		lies between	NULL		Bm-binding pocket			NULL		regions I and IV		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_3_2311_s_314	11706014	(i) When Bm-I binds to the Bm-binding pocket between regions I and IV, because the connectivity between regions III and IV is significantly strong, a significant amount of energy is necessary to cause the rotational change of region IV, which results in weak binding of Bm-I to the pocket.	bind
17401	2	5597	6	10	NULL	NULL	NULL	Bm-I	GP		bind		weakly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2311_s_314	11706014	(i) When Bm-I binds to the Bm-binding pocket between regions I and IV, because the connectivity between regions III and IV is significantly strong, a significant amount of energy is necessary to cause the rotational change of region IV, which results in weak binding of Bm-I to the pocket.	bind
16314	1	5597	7	10	NULL	NULL	NULL	Bm-I	GP		binds		weakly						Bm-binding pocket		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2311_s_314	11706014	(i) When Bm-I binds to the Bm-binding pocket between regions I and IV, because the connectivity between regions III and IV is significantly strong, a significant amount of energy is necessary to cause the rotational change of region IV, which results in weak binding of Bm-I to the pocket.	bind
16315	2	5597	7	10	NULL	NULL	NULL	statement 1	Process		occurs between								region I and IV		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2311_s_314	11706014	(i) When Bm-I binds to the Bm-binding pocket between regions I and IV, because the connectivity between regions III and IV is significantly strong, a significant amount of energy is necessary to cause the rotational change of region IV, which results in weak binding of Bm-I to the pocket.	bind
17687	1	5598	6	10	NULL	NULL	NULL	NTCB fragment	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_32182_s_210	9405419	(i) When the peptide of Met1-Pro41 was split into Met1-Gly25 and Pro26-Pro41, both peptides lost the antagonism for the actin binding of the NTCB (Fig.  4) and NN fragments (Fig.  1 c).	bind
17688	2	5598	6	10	NULL	NULL	NULL	NN fragment	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_32182_s_210	9405419	(i) When the peptide of Met1-Pro41 was split into Met1-Gly25 and Pro26-Pro41, both peptides lost the antagonism for the actin binding of the NTCB (Fig.  4) and NN fragments (Fig.  1 c).	bind
54099	3	5598	6	10	NULL	NULL	NULL	peptide	GP		split into			Met1-Pro41					Met1-Gly25		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_32182_s_210	9405419	(i) When the peptide of Met1-Pro41 was split into Met1-Gly25 and Pro26-Pro41, both peptides lost the antagonism for the actin binding of the NTCB (Fig.  4) and NN fragments (Fig.  1 c).	bind
54100	4	5598	6	10	NULL	NULL	NULL	peptide	GP		split into			Met1-Pro41					Pro26-Pro41		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_32182_s_210	9405419	(i) When the peptide of Met1-Pro41 was split into Met1-Gly25 and Pro26-Pro41, both peptides lost the antagonism for the actin binding of the NTCB (Fig.  4) and NN fragments (Fig.  1 c).	bind
54101	5	5598	6	10	NULL	NULL	NULL	statement 3	Process		loses antagonism for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_32182_s_210	9405419	(i) When the peptide of Met1-Pro41 was split into Met1-Gly25 and Pro26-Pro41, both peptides lost the antagonism for the actin binding of the NTCB (Fig.  4) and NN fragments (Fig.  1 c).	bind
54102	6	5598	6	10	NULL	NULL	NULL	statement 3	Process		loses antagonism for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_32182_s_210	9405419	(i) When the peptide of Met1-Pro41 was split into Met1-Gly25 and Pro26-Pro41, both peptides lost the antagonism for the actin binding of the NTCB (Fig.  4) and NN fragments (Fig.  1 c).	bind
54103	7	5598	6	10	NULL	NULL	NULL	statement 4	Process		loses antagonism for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_32182_s_210	9405419	(i) When the peptide of Met1-Pro41 was split into Met1-Gly25 and Pro26-Pro41, both peptides lost the antagonism for the actin binding of the NTCB (Fig.  4) and NN fragments (Fig.  1 c).	bind
54104	8	5598	6	10	NULL	NULL	NULL	statement 4	Process		loses antagonism for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_32182_s_210	9405419	(i) When the peptide of Met1-Pro41 was split into Met1-Gly25 and Pro26-Pro41, both peptides lost the antagonism for the actin binding of the NTCB (Fig.  4) and NN fragments (Fig.  1 c).	bind
16319	1	5598	7	10	NULL	NULL	NULL	actin	GP		bind					NTCB	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_32182_s_210	9405419	(i) When the peptide of Met1-Pro41 was split into Met1-Gly25 and Pro26-Pro41, both peptides lost the antagonism for the actin binding of the NTCB (Fig.  4) and NN fragments (Fig.  1 c).	bind
16320	2	5598	7	10	NULL	NULL	NULL	actin	GP		bind					NN fragments	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_32182_s_210	9405419	(i) When the peptide of Met1-Pro41 was split into Met1-Gly25 and Pro26-Pro41, both peptides lost the antagonism for the actin binding of the NTCB (Fig.  4) and NN fragments (Fig.  1 c).	bind
16321	3	5598	7	10	NULL	NULL	NULL	peptide	GP		split into			Met1-Pro41					Met1-Gly25		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_32182_s_210	9405419	(i) When the peptide of Met1-Pro41 was split into Met1-Gly25 and Pro26-Pro41, both peptides lost the antagonism for the actin binding of the NTCB (Fig.  4) and NN fragments (Fig.  1 c).	bind
16322	4	5598	7	10	NULL	NULL	NULL	peptide	GP		split into			Met1-Pro41					Pro26-Pro41		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_32182_s_210	9405419	(i) When the peptide of Met1-Pro41 was split into Met1-Gly25 and Pro26-Pro41, both peptides lost the antagonism for the actin binding of the NTCB (Fig.  4) and NN fragments (Fig.  1 c).	bind
16323	5	5598	7	10	NULL	NULL	NULL	statement 3	Process		loses					statement 1	Process	antagonism for 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_32182_s_210	9405419	(i) When the peptide of Met1-Pro41 was split into Met1-Gly25 and Pro26-Pro41, both peptides lost the antagonism for the actin binding of the NTCB (Fig.  4) and NN fragments (Fig.  1 c).	bind
16327	6	5598	7	10	NULL	NULL	NULL	statement 3	Process		loses					statement 2	Process	antagonism for 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_32182_s_210	9405419	(i) When the peptide of Met1-Pro41 was split into Met1-Gly25 and Pro26-Pro41, both peptides lost the antagonism for the actin binding of the NTCB (Fig.  4) and NN fragments (Fig.  1 c).	bind
16335	7	5598	7	10	NULL	NULL	NULL	statement 4	Process		loses					statement 1	Process	antagonism for			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_32182_s_210	9405419	(i) When the peptide of Met1-Pro41 was split into Met1-Gly25 and Pro26-Pro41, both peptides lost the antagonism for the actin binding of the NTCB (Fig.  4) and NN fragments (Fig.  1 c).	bind
16337	8	5598	7	10	NULL	NULL	NULL	statement 4	Process		loses					statement 2	Process	antagonism for 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_32182_s_210	9405419	(i) When the peptide of Met1-Pro41 was split into Met1-Gly25 and Pro26-Pro41, both peptides lost the antagonism for the actin binding of the NTCB (Fig.  4) and NN fragments (Fig.  1 c).	bind
17431	1	5599	6	10	NULL	NULL	NULL	CarS	GP		does not bind					DNA	NucleicAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_9_7262_s_8	11748235	(i) Whereas CarS exhibits no DNA binding  in vitro, CarA binds specifically to a region encompassing PB to form at least two distinct complexes.	bind
17489	2	5599	6	10	NULL	NULL	NULL	CarA	GP		bind		specifically					region encompassing		PB	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_9_7262_s_8	11748235	(i) Whereas CarS exhibits no DNA binding  in vitro, CarA binds specifically to a region encompassing PB to form at least two distinct complexes.	bind
17490	3	5599	6	10	NULL	NULL	NULL	statement 2	Process		forms 					two distinct complexes	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_9_7262_s_8	11748235	(i) Whereas CarS exhibits no DNA binding  in vitro, CarA binds specifically to a region encompassing PB to form at least two distinct complexes.	bind
16341	1	5599	7	10	NULL	NULL	NULL	CarS	GP		does not bind					DNA	NucleicAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_9_7262_s_8	11748235	(i) Whereas CarS exhibits no DNA binding  in vitro, CarA binds specifically to a region encompassing PB to form at least two distinct complexes.	bind
16342	2	5599	7	10	NULL	NULL	NULL	CarA	GP		bind		specifically					region encompassing		PB	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_9_7262_s_8	11748235	(i) Whereas CarS exhibits no DNA binding  in vitro, CarA binds specifically to a region encompassing PB to form at least two distinct complexes.	bind
16343	3	5599	7	10	NULL	NULL	NULL	statement 2	Process		forms					two distint complex	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_9_7262_s_8	11748235	(i) Whereas CarS exhibits no DNA binding  in vitro, CarA binds specifically to a region encompassing PB to form at least two distinct complexes.	bind
16344	1	5600	7	10	NULL	NULL	NULL	histidine	AminoAcid	spacing between 13residues	serve as					heme	Chemical	axial ligands for			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_14_3815_s_139	12081951	(i) Whereas the spacing (13 residues) between the histidines supposed to serve as axial ligands to the hemes is conserved in all cyt  b sequences in helix II, there are 14 residues between the heme binding histidines in helix IV in  R. gelatinosus (Fig.  4A), as already observed in cyt  b6 ( 41) and in the cyt  b subunits of the beta, gamma, and   subdivisions of proteobacteria, with the exception of  A. vinosum ( 41).	bind
16345	2	5600	7	10	NULL	NULL	NULL	statement 1	Process		is conserved in								cyt b sequences in helix II		NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_14_3815_s_139	12081951	(i) Whereas the spacing (13 residues) between the histidines supposed to serve as axial ligands to the hemes is conserved in all cyt  b sequences in helix II, there are 14 residues between the heme binding histidines in helix IV in  R. gelatinosus (Fig.  4A), as already observed in cyt  b6 ( 41) and in the cyt  b subunits of the beta, gamma, and   subdivisions of proteobacteria, with the exception of  A. vinosum ( 41).	bind
16346	3	5600	7	10	NULL	NULL	NULL			R. gelatinosus	bind			histidine in helix IV		heme	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_14_3815_s_139	12081951	(i) Whereas the spacing (13 residues) between the histidines supposed to serve as axial ligands to the hemes is conserved in all cyt  b sequences in helix II, there are 14 residues between the heme binding histidines in helix IV in  R. gelatinosus (Fig.  4A), as already observed in cyt  b6 ( 41) and in the cyt  b subunits of the beta, gamma, and   subdivisions of proteobacteria, with the exception of  A. vinosum ( 41).	bind
16347	4	5600	7	NULL	NULL	0	NULL		NULL		present in 	NULL		14 residues			NULL		histidine in helix IV		NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_14_3815_s_139	12081951	(i) Whereas the spacing (13 residues) between the histidines supposed to serve as axial ligands to the hemes is conserved in all cyt  b sequences in helix II, there are 14 residues between the heme binding histidines in helix IV in  R. gelatinosus (Fig.  4A), as already observed in cyt  b6 ( 41) and in the cyt  b subunits of the beta, gamma, and   subdivisions of proteobacteria, with the exception of  A. vinosum ( 41).	bind
17491	1	5601	6	10	NULL	NULL	NULL	DicB	GP		bind		might			MinC	GP	cytoplasmic			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_11_2951_s_263	12003935	(i) Without itself being targeted to a specific cellular location, DicB might bind cytoplasmic MinC and modify it to a form with affinity for a septal ring component.	bind
20302	2	5601	6	10	NULL	NULL	NULL	MinC	GP	modified form of;;cytoplasmic	has affinity for					septal ring component	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_11_2951_s_263	12003935	(i) Without itself being targeted to a specific cellular location, DicB might bind cytoplasmic MinC and modify it to a form with affinity for a septal ring component.	bind
20303	3	5601	6	10	NULL	NULL	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_11_2951_s_263	12003935	(i) Without itself being targeted to a specific cellular location, DicB might bind cytoplasmic MinC and modify it to a form with affinity for a septal ring component.	bind
16358	1	5601	7	10	NULL	NULL	NULL	DicB	GP		bind		might			MinC	GP	cytoplasmic			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_11_2951_s_263	12003935	(i) Without itself being targeted to a specific cellular location, DicB might bind cytoplasmic MinC and modify it to a form with affinity for a septal ring component.	bind
16359	2	5601	7	10	NULL	NULL	NULL	MinC	GP	modified form of;;cytoplasmic	has affinity for					 septal ring component	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_11_2951_s_263	12003935	(i) Without itself being targeted to a specific cellular location, DicB might bind cytoplasmic MinC and modify it to a form with affinity for a septal ring component.	bind
16360	3	5601	7	10	NULL	NULL	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_11_2951_s_263	12003935	(i) Without itself being targeted to a specific cellular location, DicB might bind cytoplasmic MinC and modify it to a form with affinity for a septal ring component.	bind
17492	1	5602	6	10	NULL	NULL	NULL	poly(L-proline)	AminoAcid		inhibits		effectively			2beta2 tetramer	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17342_s_146	9211872	(I))2beta2 tetramer is effectively inhibited by poly(L-proline) ( 1,  2) and becomes bound to poly(L-proline) affinity columns ( 20).	bind
17493	2	5602	6	10	NULL	NULL	NULL	2beta2 tetramer	GP		bind					poly(L-proline)	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17342_s_146	9211872	(I))2beta2 tetramer is effectively inhibited by poly(L-proline) ( 1,  2) and becomes bound to poly(L-proline) affinity columns ( 20).	bind
16361	1	5602	7	10	NULL	NULL	NULL	poly L-proline	AminoAcid		inhibits		effectively			2beta2 tetramer	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17342_s_146	9211872	(I))2beta2 tetramer is effectively inhibited by poly(L-proline) ( 1,  2) and becomes bound to poly(L-proline) affinity columns ( 20).	bind
16362	2	5602	7	10	NULL	NULL	NULL	2beta2 tetramer	GP		bind					poly(L-proline)	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17342_s_146	9211872	(I))2beta2 tetramer is effectively inhibited by poly(L-proline) ( 1,  2) and becomes bound to poly(L-proline) affinity columns ( 20).	bind
17494	1	5604	6	10	NULL	NULL	NULL	AcLDL	Chemical		bind					SR fusion proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_31_19592_s_193	9677385	(I), indicating that the human IgG fragment is not responsible for any of the binding of the AcLDL to the SR fusion proteins.	bind
17495	2	5604	6	10	NULL	NULL	NULL	IgG fragment	GP	human	is not responsible for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_31_19592_s_193	9677385	(I), indicating that the human IgG fragment is not responsible for any of the binding of the AcLDL to the SR fusion proteins.	bind
16363	1	5604	7	10	NULL	NULL	NULL	AcLDL	Chemical		bind					SR fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_31_19592_s_193	9677385	(I), indicating that the human IgG fragment is not responsible for any of the binding of the AcLDL to the SR fusion proteins.	bind
16364	2	5604	7	10	NULL	NULL	NULL	IgG fragment	GP	human	is not responsible for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_31_19592_s_193	9677385	(I), indicating that the human IgG fragment is not responsible for any of the binding of the AcLDL to the SR fusion proteins.	bind
17496	1	5605	6	10	NULL	NULL	NULL	C/EBP family	GP		bind					P3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_48_31629_s_27	9822619	(I), which is required for the liver-specific expression of the PEPCK gene ( 21); members of the C/EBP family are the only transcription factors that are known to bind to the P3	bind
45628	2	5605	6	10	NULL	NULL	NULL	C/EBP family	GP		is a type of					transcription factors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_48_31629_s_27	9822619	(I), which is required for the liver-specific expression of the PEPCK gene ( 21); members of the C/EBP family are the only transcription factors that are known to bind to the P3	bind
16368	1	5605	7	10	NULL	NULL	NULL	C/EBP family	GP		bind					P3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_48_31629_s_27	9822619	(I), which is required for the liver-specific expression of the PEPCK gene ( 21); members of the C/EBP family are the only transcription factors that are known to bind to the P3	bind
45629	2	5605	7	10	NULL	NULL	NULL	C/EBP family	GP		is a type of					transcription factors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_48_31629_s_27	9822619	(I), which is required for the liver-specific expression of the PEPCK gene ( 21); members of the C/EBP family are the only transcription factors that are known to bind to the P3	bind
17497	1	5609	6	10	NULL	NULL	NULL	collagen	GP		bind					alpha2beta1	GP		A-domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33287_s_241	9837901	(I)-5/6, perhaps reflecting enhancement of collagen binding to alpha2beta1 A-domain by site(s) in the adjacent EF hand domain ( 35).	bind
20304	2	5609	6	10	NULL	NULL	NULL			site adjacent to	enhance			EF hand domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33287_s_241	9837901	(I)-5/6, perhaps reflecting enhancement of collagen binding to alpha2beta1 A-domain by site(s) in the adjacent EF hand domain ( 35).	bind
16411	1	5609	7	10	NULL	NULL	NULL	collagen	GP		bind					alpha2beta1	GP		A-domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33287_s_241	9837901	(I)-5/6, perhaps reflecting enhancement of collagen binding to alpha2beta1 A-domain by site(s) in the adjacent EF hand domain ( 35).	bind
16412	2	5609	7	10	NULL	NULL	NULL			site adjacent to	enhance			EF hand domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33287_s_241	9837901	(I)-5/6, perhaps reflecting enhancement of collagen binding to alpha2beta1 A-domain by site(s) in the adjacent EF hand domain ( 35).	bind
17498	1	5610	6	10	NULL	NULL	NULL	GFOGER-GPP peptide	GP		supports 					platelet 	OrganismPart	adhesion of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_1_35_s_101	10617582	(I)-5/6-GPP, peptide GFOGER-GPP supported platelet adhesion and exhibited alpha2beta1 binding as good as that to collagen I, whereas binding of the alpha2 A-domain was consistently higher than that to the collagen (Figs.  1 and  2).	bind
17499	2	5610	6	10	NULL	NULL	NULL	GFOGER-GPP peptide	GP		bind					alpha2beta1 	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_1_35_s_101	10617582	(I)-5/6-GPP, peptide GFOGER-GPP supported platelet adhesion and exhibited alpha2beta1 binding as good as that to collagen I, whereas binding of the alpha2 A-domain was consistently higher than that to the collagen (Figs.  1 and  2).	bind
17500	3	5610	6	10	NULL	NULL	NULL	GFOGER-GPP peptide	GP		bind					collagen I	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_1_35_s_101	10617582	(I)-5/6-GPP, peptide GFOGER-GPP supported platelet adhesion and exhibited alpha2beta1 binding as good as that to collagen I, whereas binding of the alpha2 A-domain was consistently higher than that to the collagen (Figs.  1 and  2).	bind
17728	4	5610	6	10	NULL	NULL	NULL	statement 2	Process		is as good as					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_1_35_s_101	10617582	(I)-5/6-GPP, peptide GFOGER-GPP supported platelet adhesion and exhibited alpha2beta1 binding as good as that to collagen I, whereas binding of the alpha2 A-domain was consistently higher than that to the collagen (Figs.  1 and  2).	bind
17729	5	5610	6	10	NULL	NULL	NULL	GFOGER-GPP peptide	GP		bind					alpha 2	GP		A-domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_1_35_s_101	10617582	(I)-5/6-GPP, peptide GFOGER-GPP supported platelet adhesion and exhibited alpha2beta1 binding as good as that to collagen I, whereas binding of the alpha2 A-domain was consistently higher than that to the collagen (Figs.  1 and  2).	bind
17730	6	5610	6	10	NULL	NULL	NULL	statement 5	Process		is higher than					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_1_35_s_101	10617582	(I)-5/6-GPP, peptide GFOGER-GPP supported platelet adhesion and exhibited alpha2beta1 binding as good as that to collagen I, whereas binding of the alpha2 A-domain was consistently higher than that to the collagen (Figs.  1 and  2).	bind
16413	1	5610	7	10	NULL	NULL	NULL	GFOGER-GPP peptide	GP		support					platelets	OrganismPart	adhesion of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_1_35_s_101	10617582	(I)-5/6-GPP, peptide GFOGER-GPP supported platelet adhesion and exhibited alpha2beta1 binding as good as that to collagen I, whereas binding of the alpha2 A-domain was consistently higher than that to the collagen (Figs.  1 and  2).	bind
16414	2	5610	7	10	NULL	NULL	NULL	GFOGER-GPP peptide	GP		bind					alpha2beta1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_1_35_s_101	10617582	(I)-5/6-GPP, peptide GFOGER-GPP supported platelet adhesion and exhibited alpha2beta1 binding as good as that to collagen I, whereas binding of the alpha2 A-domain was consistently higher than that to the collagen (Figs.  1 and  2).	bind
16415	3	5610	7	10	NULL	NULL	NULL	GFOGER-GPP peptide	GP		bind					collagen I	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_1_35_s_101	10617582	(I)-5/6-GPP, peptide GFOGER-GPP supported platelet adhesion and exhibited alpha2beta1 binding as good as that to collagen I, whereas binding of the alpha2 A-domain was consistently higher than that to the collagen (Figs.  1 and  2).	bind
16416	4	5610	7	10	NULL	NULL	NULL	GFOGER-GPP peptide	GP		bind					alpha2	GP		A-domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_1_35_s_101	10617582	(I)-5/6-GPP, peptide GFOGER-GPP supported platelet adhesion and exhibited alpha2beta1 binding as good as that to collagen I, whereas binding of the alpha2 A-domain was consistently higher than that to the collagen (Figs.  1 and  2).	bind
16417	5	5610	7	10	NULL	NULL	NULL	statement 2	Process		is as good as					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_1_35_s_101	10617582	(I)-5/6-GPP, peptide GFOGER-GPP supported platelet adhesion and exhibited alpha2beta1 binding as good as that to collagen I, whereas binding of the alpha2 A-domain was consistently higher than that to the collagen (Figs.  1 and  2).	bind
16418	6	5610	7	10	NULL	NULL	NULL	GFOGER-GPP peptide	GP		bind					collagen	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_1_35_s_101	10617582	(I)-5/6-GPP, peptide GFOGER-GPP supported platelet adhesion and exhibited alpha2beta1 binding as good as that to collagen I, whereas binding of the alpha2 A-domain was consistently higher than that to the collagen (Figs.  1 and  2).	bind
16419	7	5610	7	10	NULL	NULL	NULL	statement 4	Process		is higher than					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_1_35_s_101	10617582	(I)-5/6-GPP, peptide GFOGER-GPP supported platelet adhesion and exhibited alpha2beta1 binding as good as that to collagen I, whereas binding of the alpha2 A-domain was consistently higher than that to the collagen (Figs.  1 and  2).	bind
17501	1	5611	6	10	NULL	NULL	NULL	IL-2	GP		bind					Collagen	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_49_38170_s_110	10982811	(I)-derived CNBr Peptides Inhibit Binding of IL-2 to Immobilized Collagen-- Incubation of IL-2 with the constituent chains of collagen type I, namely alpha1 and alpha2, with native collagen types III and IV, previously immobilized at 50 ng/200 mul/well, in the presence of increasing amounts of solubilized collagen chains or their CNBr peptides resulted in a dose-dependent inhibition of the IL-2-collagen interaction.	bind
17502	2	5611	6	10	NULL	NULL	NULL	CNBr peptides	GP		inhibits		dose dependently			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_49_38170_s_110	10982811	(I)-derived CNBr Peptides Inhibit Binding of IL-2 to Immobilized Collagen-- Incubation of IL-2 with the constituent chains of collagen type I, namely alpha1 and alpha2, with native collagen types III and IV, previously immobilized at 50 ng/200 mul/well, in the presence of increasing amounts of solubilized collagen chains or their CNBr peptides resulted in a dose-dependent inhibition of the IL-2-collagen interaction.	bind
16420	1	5611	7	10	NULL	NULL	NULL	IL-2	GP		bind					Collagen	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_49_38170_s_110	10982811	(I)-derived CNBr Peptides Inhibit Binding of IL-2 to Immobilized Collagen-- Incubation of IL-2 with the constituent chains of collagen type I, namely alpha1 and alpha2, with native collagen types III and IV, previously immobilized at 50 ng/200 mul/well, in the presence of increasing amounts of solubilized collagen chains or their CNBr peptides resulted in a dose-dependent inhibition of the IL-2-collagen interaction.	bind
16421	2	5611	7	10	NULL	NULL	NULL	CNBr Peptides	GP		inhibits		dose-dependently			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_49_38170_s_110	10982811	(I)-derived CNBr Peptides Inhibit Binding of IL-2 to Immobilized Collagen-- Incubation of IL-2 with the constituent chains of collagen type I, namely alpha1 and alpha2, with native collagen types III and IV, previously immobilized at 50 ng/200 mul/well, in the presence of increasing amounts of solubilized collagen chains or their CNBr peptides resulted in a dose-dependent inhibition of the IL-2-collagen interaction.	bind
17503	1	5612	6	10	NULL	NULL	NULL				bind			RBD		GST-L18	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_2_1116_s_156	9891046	(I)-poly(C) (5 and 15 mug/ml) significantly reduced the amount of RBD bound to GST-L18 (Fig.  3A, lanes 2 and 3).	bind
17504	2	5612	6	10	NULL	NULL	NULL	poly(C)	Chemical		reduces		significantly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_2_1116_s_156	9891046	(I)-poly(C) (5 and 15 mug/ml) significantly reduced the amount of RBD bound to GST-L18 (Fig.  3A, lanes 2 and 3).	bind
16422	1	5612	7	10	NULL	NULL	NULL				bind			RBD		GST-L18	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_2_1116_s_156	9891046	(I)-poly(C) (5 and 15 mug/ml) significantly reduced the amount of RBD bound to GST-L18 (Fig.  3A, lanes 2 and 3).	bind
16423	2	5612	7	10	NULL	NULL	NULL	poly(C)	Chemical		reduces		significantly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_2_1116_s_156	9891046	(I)-poly(C) (5 and 15 mug/ml) significantly reduced the amount of RBD bound to GST-L18 (Fig.  3A, lanes 2 and 3).	bind
17505	1	5615	6	10	NULL	NULL	NULL	THP	GP		bind			127 - 138		alpha2 integrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_33_30516_s_199	12788934	(I)127 - 138 THP bound  7  times more strongly to the alpha2 integrin subunit than to  alpha1beta1 integrins or  alphaVbeta3 integrins, which had equivalent binding  strengths.	bind
17506	2	5615	6	10	NULL	NULL	NULL	THP	GP		bind			127 - 138		alpha1beta1 integrins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_33_30516_s_199	12788934	(I)127 - 138 THP bound  7  times more strongly to the alpha2 integrin subunit than to  alpha1beta1 integrins or  alphaVbeta3 integrins, which had equivalent binding  strengths.	bind
17507	3	5615	6	10	NULL	NULL	NULL	THP	GP		bind			127 - 138		alphaVbeta3 integrins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_33_30516_s_199	12788934	(I)127 - 138 THP bound  7  times more strongly to the alpha2 integrin subunit than to  alpha1beta1 integrins or  alphaVbeta3 integrins, which had equivalent binding  strengths.	bind
17508	4	5615	6	10	NULL	NULL	NULL	statement 1	Process		is stronger than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_33_30516_s_199	12788934	(I)127 - 138 THP bound  7  times more strongly to the alpha2 integrin subunit than to  alpha1beta1 integrins or  alphaVbeta3 integrins, which had equivalent binding  strengths.	bind
17509	5	5615	6	10	NULL	NULL	NULL	statement 1	Process		is stronger than					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_33_30516_s_199	12788934	(I)127 - 138 THP bound  7  times more strongly to the alpha2 integrin subunit than to  alpha1beta1 integrins or  alphaVbeta3 integrins, which had equivalent binding  strengths.	bind
20305	6	5615	6	10	NULL	NULL	NULL	statement 2	Process		has equivalent strength to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_33_30516_s_199	12788934	(I)127 - 138 THP bound  7  times more strongly to the alpha2 integrin subunit than to  alpha1beta1 integrins or  alphaVbeta3 integrins, which had equivalent binding  strengths.	bind
16426	1	5615	7	10	NULL	NULL	NULL	THP	GP		bind			127 - 138		alpha2 integrin subunit	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_33_30516_s_199	12788934	(I)127 - 138 THP bound  7  times more strongly to the alpha2 integrin subunit than to  alpha1beta1 integrins or  alphaVbeta3 integrins, which had equivalent binding  strengths.	bind
16427	2	5615	7	10	NULL	NULL	NULL	THP	GP		bind			127 - 138		alpha1beta1 integrins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_33_30516_s_199	12788934	(I)127 - 138 THP bound  7  times more strongly to the alpha2 integrin subunit than to  alpha1beta1 integrins or  alphaVbeta3 integrins, which had equivalent binding  strengths.	bind
16428	3	5615	7	10	NULL	NULL	NULL	THP	GP		bind			127 - 138		alphaVbeta3 integrins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_33_30516_s_199	12788934	(I)127 - 138 THP bound  7  times more strongly to the alpha2 integrin subunit than to  alpha1beta1 integrins or  alphaVbeta3 integrins, which had equivalent binding  strengths.	bind
16429	4	5615	7	10	NULL	NULL	NULL	statement 1	Process		is stronger than		significantly			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_33_30516_s_199	12788934	(I)127 - 138 THP bound  7  times more strongly to the alpha2 integrin subunit than to  alpha1beta1 integrins or  alphaVbeta3 integrins, which had equivalent binding  strengths.	bind
16430	5	5615	7	10	NULL	NULL	NULL	statement 1	Process		is stronger than		significantly			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_33_30516_s_199	12788934	(I)127 - 138 THP bound  7  times more strongly to the alpha2 integrin subunit than to  alpha1beta1 integrins or  alphaVbeta3 integrins, which had equivalent binding  strengths.	bind
16431	6	5615	7	10	NULL	NULL	NULL	statement 2	Process		has equivalent strength to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_33_30516_s_199	12788934	(I)127 - 138 THP bound  7  times more strongly to the alpha2 integrin subunit than to  alpha1beta1 integrins or  alphaVbeta3 integrins, which had equivalent binding  strengths.	bind
17510	1	5616	6	10	NULL	NULL	NULL	THP	GP		bind		high affinity	925-937		heparin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_13_7275_s_121	9636139	(I)925-937 THP bound heparin with high affinity.	bind
16432	1	5616	7	10	NULL	NULL	NULL	THP	GP		bind		high affinity	925-937		heparin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_13_7275_s_121	9636139	(I)925-937 THP bound heparin with high affinity.	bind
17511	1	5617	6	10	NULL	NULL	NULL	THP	GP		bind		tightly	925-937		medium Mr heparin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_13_7275_s_101	9636139	(I)925-937 THP or type I collagen bound even more tightly to medium  Mr heparin ( Kd   250 nM and 14 nM, respectively).	bind
17512	2	5617	6	10	NULL	NULL	NULL	type I collagen	GP		bind		tightly			medium Mr heparin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_13_7275_s_101	9636139	(I)925-937 THP or type I collagen bound even more tightly to medium  Mr heparin ( Kd   250 nM and 14 nM, respectively).	bind
16433	1	5617	7	10	NULL	NULL	NULL	THP	GP		bind		tightly	925-937		medium Mr heparin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_13_7275_s_101	9636139	(I)925-937 THP or type I collagen bound even more tightly to medium  Mr heparin ( Kd   250 nM and 14 nM, respectively).	bind
16434	2	5617	7	10	NULL	NULL	NULL	 type I collagen	GP		bind		tightly			medium Mr heparin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_13_7275_s_101	9636139	(I)925-937 THP or type I collagen bound even more tightly to medium  Mr heparin ( Kd   250 nM and 14 nM, respectively).	bind
17513	1	5618	6	10	NULL	NULL	NULL	TLR3	GP	WT	bind		directly	ECD		pI:pC	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_23_8792_s_79	16720699	(I):p(C), a major portion of WT TLR3-ECD elutes in the void volume, at the same position as pI:pC (fraction 4), indicating that WT TLR3-ECD directly binds pI:pC.	bind
16435	1	5618	7	10	NULL	NULL	NULL	TLR3	GP	WT	binds		directly	ECD		pI:pC	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_23_8792_s_79	16720699	(I):p(C), a major portion of WT TLR3-ECD elutes in the void volume, at the same position as pI:pC (fraction 4), indicating that WT TLR3-ECD directly binds pI:pC.	bind
17521	1	5620	6	10	NULL	NULL	NULL	TnI	GP	skeletal	bind			residues 128-148		actin-tropomyosin	GP				NULL		NULL	NULL	NULL	NULL	gw70_nature_424_6944_35_s_163	12840750	(I); the corresponding peptide (residues 128-148  in skeletal TnI) binds to actin-tropomyosin and induces a weak inhibitory activity  on its own 32.	bind
16436	1	5620	7	10	NULL	NULL	NULL	 TnI	GP	skeletal	bind			128-148		actin-tropomyosin	GP				NULL		NULL	NULL	NULL	NULL	gw70_nature_424_6944_35_s_163	12840750	(I); the corresponding peptide (residues 128-148  in skeletal TnI) binds to actin-tropomyosin and induces a weak inhibitory activity  on its own 32.	bind
17522	1	5621	6	10	NULL	NULL	NULL	eutT genes	GP		encode					adenosyl-transferases	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_49_40948_s_24	16207720	(I)alamin adenosyl-transferases encoded by the  eutT and  pduO genes ( - ).	bind
17523	2	5621	6	10	NULL	NULL	NULL	pduO genes	GP		encode					adenosyl-transferases	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_49_40948_s_24	16207720	(I)alamin adenosyl-transferases encoded by the  eutT and  pduO genes ( - ).	bind
16438	1	5621	7	10	NULL	NULL	NULL	eutT gene	GP		encode					alamin adenosyl-transferases	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_49_40948_s_24	16207720	(I)alamin adenosyl-transferases encoded by the  eutT and  pduO genes ( - ).	bind
16439	2	5621	7	10	NULL	NULL	NULL	pduO gene	GP		encode					alamin adenosyl-transferases	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_49_40948_s_24	16207720	(I)alamin adenosyl-transferases encoded by the  eutT and  pduO genes ( - ).	bind
17524	1	5622	6	10	NULL	NULL	NULL	amide	Chemical		bind					CoFeSPCh	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_39_14331_s_166	16983091	(I)amide bound to CoFeSPCh and CH3-H4folate bound to MeTr.	bind
17525	2	5622	6	10	NULL	NULL	NULL	MeTr	GP		bind					CH3-H4folate	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_39_14331_s_166	16983091	(I)amide bound to CoFeSPCh and CH3-H4folate bound to MeTr.	bind
16440	1	5622	7	10	NULL	NULL	NULL	amide	Chemical		bind					CoFeSPCh	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_39_14331_s_166	16983091	(I)amide bound to CoFeSPCh and CH3-H4folate bound to MeTr.	bind
16441	2	5622	7	10	NULL	NULL	NULL	CH3-H4folate	Chemical		bind					MeTr 	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_39_14331_s_166	16983091	(I)amide bound to CoFeSPCh and CH3-H4folate bound to MeTr.	bind
17526	1	5623	6	10	NULL	NULL	NULL	collagen type I	GP		bind			CB6		heparin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_3_1613_s_8	8576160	(I)CB6 of collagen type I, which also  binds heparin.	bind
16442	1	5623	7	10	NULL	NULL	NULL	type I collagen	GP		bind			CB6		heparin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_3_1613_s_8	8576160	(I)CB6 of collagen type I, which also  binds heparin.	bind
17527	1	5624	6	10	NULL	NULL	NULL	KGF	GP		bind					alpha1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_30_26872_s_121	11973338	(I)CB8 as inhibitors of KGF binding to alpha1	bind
20306	2	5624	6	10	NULL	NULL	NULL	CB8	Chemical		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_30_26872_s_121	11973338	(I)CB8 as inhibitors of KGF binding to alpha1	bind
16443	1	5624	7	10	NULL	NULL	NULL	KGF	GP		bind					alpha1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_30_26872_s_121	11973338	(I)CB8 as inhibitors of KGF binding to alpha1	bind
16444	2	5624	7	10	NULL	NULL	NULL	CB8	Chemical		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_30_26872_s_121	11973338	(I)CB8 as inhibitors of KGF binding to alpha1	bind
17528	1	5625	6	10	NULL	NULL	NULL	Dkk-1-AP	GP		bind					LRP6N-IgG	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_90	11448771	(I, II) or hIgG (III, IV) Abs.  (c) Dkk-1-AP binding to LRP6N-IgG (circles, line) or IgG (squares).	bind
17529	2	5625	6	10	NULL	NULL	NULL	Dkk-1-AP	GP		bind					IgG	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_90	11448771	(I, II) or hIgG (III, IV) Abs.  (c) Dkk-1-AP binding to LRP6N-IgG (circles, line) or IgG (squares).	bind
17530	3	5625	6	10	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_90	11448771	(I, II) or hIgG (III, IV) Abs.  (c) Dkk-1-AP binding to LRP6N-IgG (circles, line) or IgG (squares).	bind
16445	1	5625	7	10	NULL	NULL	NULL	Dkk-1-AP	GP		bind					LRP6N-IgG	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_90	11448771	(I, II) or hIgG (III, IV) Abs.  (c) Dkk-1-AP binding to LRP6N-IgG (circles, line) or IgG (squares).	bind
20275	2	5625	7	10	NULL	NULL	NULL	Dkk-1-AP	GP		bind					IgG	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_90	11448771	(I, II) or hIgG (III, IV) Abs.  (c) Dkk-1-AP binding to LRP6N-IgG (circles, line) or IgG (squares).	bind
20276	3	5625	7	10	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_90	11448771	(I, II) or hIgG (III, IV) Abs.  (c) Dkk-1-AP binding to LRP6N-IgG (circles, line) or IgG (squares).	bind
17531	1	5627	6	10	NULL	NULL	NULL	pCVI-HSA	GP		bind					HSC	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_17_12743_s_275	10777570	(I, III, VI, and IV) interfered with 125I-pCVI-HSA binding to HSC (data not shown).	bind
16447	1	5627	7	10	NULL	NULL	NULL	25I-pCVI-HSA	GP		bind					HSC	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_17_12743_s_275	10777570	(I, III, VI, and IV) interfered with 125I-pCVI-HSA binding to HSC (data not shown).	bind
17685	1	5628	6	10	NULL	NULL	NULL	p12I	GP		bind		may			calcineurin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_18_15550_s_122	12601010	(I/ L)T Binds Calcineurin To test whether p12I binds calcineurin, we transiently transfected p12I into both 293T and Jurkat T cells and performed both immunoprecipitation and calmodulin bead pull-down experiments (Fig.  2).	bind
25321	1	5628	7	10	NULL	NULL	NULL	p12I	GP		bind		may			calcineurin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_18_15550_s_122	12601010	(I/ L)T Binds Calcineurin To test whether p12I binds calcineurin, we transiently transfected p12I into both 293T and Jurkat T cells and performed both immunoprecipitation and calmodulin bead pull-down experiments (Fig.  2).	bind
17693	1	5629	6	10	NULL	NULL	NULL	CXCL9	GP		bind					memory CD8+ T cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_9_2456_s_170	16955143	(I:C) diminished staining of CXCR3 on memory CD8+ T cells (Figure  3E), suggesting binding of its ligand CXCL9 and consequent downregulation of CXCR3 ( ).	bind
45748	2	5629	6	10	NULL	NULL	NULL	statement 1	Process		downregulates					CXCR3	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_9_2456_s_170	16955143	(I:C) diminished staining of CXCR3 on memory CD8+ T cells (Figure  3E), suggesting binding of its ligand CXCL9 and consequent downregulation of CXCR3 ( ).	bind
17023	1	5629	7	10	NULL	NULL	NULL	CXCL9	GP		bind					memory CD8+ T cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_9_2456_s_170	16955143	(I:C) diminished staining of CXCR3 on memory CD8+ T cells (Figure  3E), suggesting binding of its ligand CXCL9 and consequent downregulation of CXCR3 ( ).	bind
17024	2	5629	7	10	NULL	NULL	NULL	statement 1	Process		downregulates					CXCR3 	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_9_2456_s_170	16955143	(I:C) diminished staining of CXCR3 on memory CD8+ T cells (Figure  3E), suggesting binding of its ligand CXCL9 and consequent downregulation of CXCR3 ( ).	bind
17695	1	5630	6	10	NULL	NULL	NULL	TRIF-TRAF6	GP		play a role in					TAK1	GP	activation of 			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_22_2668_s_106	16260493	(I:C) leads to TAK1 activation through TRIF - TRAF6 (Sato et al. 2003 ), followed by NF-kappaB activation (Jiang et al. 2003 ).	bind
20307	2	5630	6	10	NULL	NULL	NULL	statement 1	Process		is followed by					NF-kappaB	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_22_2668_s_106	16260493	(I:C) leads to TAK1 activation through TRIF - TRAF6 (Sato et al. 2003 ), followed by NF-kappaB activation (Jiang et al. 2003 ).	bind
17025	1	5630	7	10	NULL	NULL	NULL	TAK1	GP	activation of	occurs through					TRIF - TRAF6	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_22_2668_s_106	16260493	(I:C) leads to TAK1 activation through TRIF - TRAF6 (Sato et al. 2003 ), followed by NF-kappaB activation (Jiang et al. 2003 ).	bind
17026	2	5630	7	10	NULL	NULL	NULL	statement 1	Process		is followed by					NF-kappaB	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_22_2668_s_106	16260493	(I:C) leads to TAK1 activation through TRIF - TRAF6 (Sato et al. 2003 ), followed by NF-kappaB activation (Jiang et al. 2003 ).	bind
17696	1	5632	6	10	NULL	NULL	NULL	IFN-inducing factor	GP		induces					IL-8	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_8_867_s_406	10222332	(IFN-inducing factor) induces IL-8 and IL-1 via TNF production from non-CD14+ human blood mononuclear cells.	bind
17697	2	5632	6	10	NULL	NULL	NULL	IFN-inducing factor	GP		induces					IL-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_8_867_s_406	10222332	(IFN-inducing factor) induces IL-8 and IL-1 via TNF production from non-CD14+ human blood mononuclear cells.	bind
17698	3	5632	6	10	NULL	NULL	NULL	blood mononuclear cells	Cell	non-CD14+ human	produce					TNF	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_8_867_s_406	10222332	(IFN-inducing factor) induces IL-8 and IL-1 via TNF production from non-CD14+ human blood mononuclear cells.	bind
17699	4	5632	6	10	NULL	NULL	NULL	statement 1	Process		occurs via					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_8_867_s_406	10222332	(IFN-inducing factor) induces IL-8 and IL-1 via TNF production from non-CD14+ human blood mononuclear cells.	bind
17700	5	5632	6	10	NULL	NULL	NULL	statement 2	Process		occurs via					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_8_867_s_406	10222332	(IFN-inducing factor) induces IL-8 and IL-1 via TNF production from non-CD14+ human blood mononuclear cells.	bind
17027	1	5632	7	10	NULL	NULL	NULL	IFN-inducing factor	GP		induce					IL-8	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_8_867_s_406	10222332	(IFN-inducing factor) induces IL-8 and IL-1 via TNF production from non-CD14+ human blood mononuclear cells.	bind
17028	2	5632	7	10	NULL	NULL	NULL	IFN-inducing factor	GP		induce					IL-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_8_867_s_406	10222332	(IFN-inducing factor) induces IL-8 and IL-1 via TNF production from non-CD14+ human blood mononuclear cells.	bind
17029	4	5632	7	10	NULL	NULL	NULL	statement 1	Process		occurs via					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_8_867_s_406	10222332	(IFN-inducing factor) induces IL-8 and IL-1 via TNF production from non-CD14+ human blood mononuclear cells.	bind
17030	5	5632	7	10	NULL	NULL	NULL	statement 2	Process		occurs via					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_8_867_s_406	10222332	(IFN-inducing factor) induces IL-8 and IL-1 via TNF production from non-CD14+ human blood mononuclear cells.	bind
45836	3	5632	7	10	NULL	NULL	NULL	blood mononuclear cells	Cell	non-CD14+ human	produce					TNF	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_8_867_s_406	10222332	(IFN-inducing factor) induces IL-8 and IL-1 via TNF production from non-CD14+ human blood mononuclear cells.	bind
17701	1	5633	6	10	NULL	NULL	NULL	FK506 peptidomacrolide	Chemical		bind					PP2B	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_97_1_21_s_9	11744159	(ii) After complexation with FKBP12, the FK506 peptidomacrolide binds to the protein phosphatase calcineurin (PP2B) which results in immediate inhibition of calcineurin activity.	bind
17702	2	5633	6	10	NULL	NULL	NULL	PP2B	GP		is					protein phosphatase calcineurin 	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_97_1_21_s_9	11744159	(ii) After complexation with FKBP12, the FK506 peptidomacrolide binds to the protein phosphatase calcineurin (PP2B) which results in immediate inhibition of calcineurin activity.	bind
17703	3	5633	6	10	NULL	NULL	NULL	statement 1	Process		inhibits					calcineurin 	GP	activity of 			NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_97_1_21_s_9	11744159	(ii) After complexation with FKBP12, the FK506 peptidomacrolide binds to the protein phosphatase calcineurin (PP2B) which results in immediate inhibition of calcineurin activity.	bind
17704	4	5633	6	10	NULL	NULL	NULL	FK506 peptidomacrolide	Chemical		complexes with					FKBP12	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_97_1_21_s_9	11744159	(ii) After complexation with FKBP12, the FK506 peptidomacrolide binds to the protein phosphatase calcineurin (PP2B) which results in immediate inhibition of calcineurin activity.	bind
17705	5	5633	6	10	NULL	NULL	NULL	statement 1	Process		occurs after					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_97_1_21_s_9	11744159	(ii) After complexation with FKBP12, the FK506 peptidomacrolide binds to the protein phosphatase calcineurin (PP2B) which results in immediate inhibition of calcineurin activity.	bind
17031	1	5633	7	10	NULL	NULL	NULL	FK506 peptidomacrolide	Chemical		complex with					FKBP12	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_97_1_21_s_9	11744159	(ii) After complexation with FKBP12, the FK506 peptidomacrolide binds to the protein phosphatase calcineurin (PP2B) which results in immediate inhibition of calcineurin activity.	bind
17032	2	5633	7	10	NULL	NULL	NULL	FK506 peptidomacrolide	Chemical		binds to					PP2B	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_97_1_21_s_9	11744159	(ii) After complexation with FKBP12, the FK506 peptidomacrolide binds to the protein phosphatase calcineurin (PP2B) which results in immediate inhibition of calcineurin activity.	bind
17033	3	5633	7	10	NULL	NULL	NULL	statement 2	Process		occurs after					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_97_1_21_s_9	11744159	(ii) After complexation with FKBP12, the FK506 peptidomacrolide binds to the protein phosphatase calcineurin (PP2B) which results in immediate inhibition of calcineurin activity.	bind
17034	4	5633	7	10	NULL	NULL	NULL	statement 2	Process		inhibits					calcineurin	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_97_1_21_s_9	11744159	(ii) After complexation with FKBP12, the FK506 peptidomacrolide binds to the protein phosphatase calcineurin (PP2B) which results in immediate inhibition of calcineurin activity.	bind
17035	5	5633	7	10	NULL	NULL	NULL	PP2B	GP		is					protein phosphatase calcineurin	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_97_1_21_s_9	11744159	(ii) After complexation with FKBP12, the FK506 peptidomacrolide binds to the protein phosphatase calcineurin (PP2B) which results in immediate inhibition of calcineurin activity.	bind
17706	1	5634	6	10	NULL	NULL	NULL	ATP	Chemical	hydrolysis of	unwraps					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_601_s_229	11157766	(ii) After the ATP hydrolysis the DNA becomes unwrapped, but UvrA remains bound to the complex, thereby directing the wrapping after binding of the new ATP molecule.	bind
17707	2	5634	6	10	NULL	NULL	NULL	UvrA	GP		directs					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_601_s_229	11157766	(ii) After the ATP hydrolysis the DNA becomes unwrapped, but UvrA remains bound to the complex, thereby directing the wrapping after binding of the new ATP molecule.	bind
17708	3	5634	6	10	NULL	NULL	NULL	statement 2	Process		occurs after					ATP molecule	Chemical	wrapping of 			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_601_s_229	11157766	(ii) After the ATP hydrolysis the DNA becomes unwrapped, but UvrA remains bound to the complex, thereby directing the wrapping after binding of the new ATP molecule.	bind
17036	1	5634	7	10	NULL	NULL	NULL	ATP	Chemical	hydrolysis of	unwraps					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_601_s_229	11157766	(ii) After the ATP hydrolysis the DNA becomes unwrapped, but UvrA remains bound to the complex, thereby directing the wrapping after binding of the new ATP molecule.	bind
17037	3	5634	7	10	NULL	NULL	NULL	UvrA	GP		directs					DNA	NucleicAcid	wrapping of			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_601_s_229	11157766	(ii) After the ATP hydrolysis the DNA becomes unwrapped, but UvrA remains bound to the complex, thereby directing the wrapping after binding of the new ATP molecule.	bind
17038	2	5634	7	10	NULL	NULL	NULL	statement 1	Process		bind					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_601_s_229	11157766	(ii) After the ATP hydrolysis the DNA becomes unwrapped, but UvrA remains bound to the complex, thereby directing the wrapping after binding of the new ATP molecule.	bind
20285	4	5634	7	10	NULL	NULL	NULL	statement 3	Process		occurs after					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_601_s_229	11157766	(ii) After the ATP hydrolysis the DNA becomes unwrapped, but UvrA remains bound to the complex, thereby directing the wrapping after binding of the new ATP molecule.	bind
17709	1	5635	6	10	NULL	NULL	NULL	HSF	GP		bind									HSE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_28_26332_s_238	11306579	(ii) Alternatively, it could be recruited only when HSFs binds to the HSEs and increase the stability of the nucleoprotein complex (Fig.  7 B).	bind
17710	2	5635	6	10	NULL	NULL	NULL	statement 1	Process		increase					nucleoprotein complex	GP	stability of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_28_26332_s_238	11306579	(ii) Alternatively, it could be recruited only when HSFs binds to the HSEs and increase the stability of the nucleoprotein complex (Fig.  7 B).	bind
17041	1	5635	7	10	NULL	NULL	NULL	HSF	GP		bind									HSE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_28_26332_s_238	11306579	(ii) Alternatively, it could be recruited only when HSFs binds to the HSEs and increase the stability of the nucleoprotein complex (Fig.  7 B).	bind
17042	2	5635	7	10	NULL	NULL	NULL	statement 1	Process		increase					nucleoprotein complex	GP	stability of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_28_26332_s_238	11306579	(ii) Alternatively, it could be recruited only when HSFs binds to the HSEs and increase the stability of the nucleoprotein complex (Fig.  7 B).	bind
20739	1	5636	6	10	NULL	NULL	NULL	OP2	GP		allow		could			unidentified regulator protein	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_19_5948_s_158	10498706	(ii) Alternatively, OP2 could allow the binding of an unidentified regulator protein acting synergically with KdgR and whose action would strictly depend on the simultaneous presence of KdgR.	bind
20740	2	5636	6	10	NULL	NULL	NULL	unidentified regulator protein	GP		acts with		synergistically			KdgR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_19_5948_s_158	10498706	(ii) Alternatively, OP2 could allow the binding of an unidentified regulator protein acting synergically with KdgR and whose action would strictly depend on the simultaneous presence of KdgR.	bind
20741	3	5636	6	10	NULL	NULL	NULL	unidentified regulator protein	GP	action of	depend on		strictly;; could			KdgR	GP	presence of 			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_19_5948_s_158	10498706	(ii) Alternatively, OP2 could allow the binding of an unidentified regulator protein acting synergically with KdgR and whose action would strictly depend on the simultaneous presence of KdgR.	bind
17043	1	5636	7	10	NULL	NULL	NULL	OP2	GP		allows					unidentified regulator protein 	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_19_5948_s_158	10498706	(ii) Alternatively, OP2 could allow the binding of an unidentified regulator protein acting synergically with KdgR and whose action would strictly depend on the simultaneous presence of KdgR.	bind
17050	2	5636	7	10	NULL	NULL	NULL	unidentified regulator protein 	GP		acts		synergistically			KdgR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_19_5948_s_158	10498706	(ii) Alternatively, OP2 could allow the binding of an unidentified regulator protein acting synergically with KdgR and whose action would strictly depend on the simultaneous presence of KdgR.	bind
17051	3	5636	7	10	NULL	NULL	NULL	unidentified regulator protein 	GP	action of	depends on		strictly			KdgR	GP	presence of			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_19_5948_s_158	10498706	(ii) Alternatively, OP2 could allow the binding of an unidentified regulator protein acting synergically with KdgR and whose action would strictly depend on the simultaneous presence of KdgR.	bind
17711	1	5637	6	10	NULL	NULL	NULL	CaM	GP		blocks 		completely			G protein	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_42_32672_s_340	10926927	(ii) At a concentration where CaM completely blocks G protein activation, the formation of the agonist/receptor/G protein complex, hence, high affinity agonist binding is virtually unaffected.	bind
20308	2	5637	6	10	NULL	NULL	NULL	CaM	GP		does not affect					agonist/receptor/G protein complex	GP	formation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_42_32672_s_340	10926927	(ii) At a concentration where CaM completely blocks G protein activation, the formation of the agonist/receptor/G protein complex, hence, high affinity agonist binding is virtually unaffected.	bind
20309	3	5637	6	10	NULL	NULL	NULL	CaM	GP		does not affect					agonist	GP	high affinity binding of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_42_32672_s_340	10926927	(ii) At a concentration where CaM completely blocks G protein activation, the formation of the agonist/receptor/G protein complex, hence, high affinity agonist binding is virtually unaffected.	bind
17052	1	5637	7	10	NULL	NULL	NULL	CaM	GP		blocks		completely			G protein	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_42_32672_s_340	10926927	(ii) At a concentration where CaM completely blocks G protein activation, the formation of the agonist/receptor/G protein complex, hence, high affinity agonist binding is virtually unaffected.	bind
17053	2	5637	7	10	NULL	NULL	NULL	CaM	GP		does not affect					agonist/receptor/G protein complex	GP	formation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_42_32672_s_340	10926927	(ii) At a concentration where CaM completely blocks G protein activation, the formation of the agonist/receptor/G protein complex, hence, high affinity agonist binding is virtually unaffected.	bind
17056	3	5637	7	10	NULL	NULL	NULL	CaM	GP		does not affect					agonist	GP	high affinity binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_42_32672_s_340	10926927	(ii) At a concentration where CaM completely blocks G protein activation, the formation of the agonist/receptor/G protein complex, hence, high affinity agonist binding is virtually unaffected.	bind
17712	1	5638	6	10	NULL	NULL	NULL	ATP	Chemical		bind					polypeptide-containing ring of GroEL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_30_21251_s_20	10409682	(ii) Bind-ing of ATP to the polypeptide-containing ring of GroEL permits the binding of GroES to that ring accompanying the release of polypeptide into an enclosed cage, defined by the GroEL cavity and the dome of GroES, in which folding to the native state can proceed with aggregation being avoided ( 6,  8-13).	bind
17713	2	5638	6	10	NULL	NULL	NULL	GroES	GP		bind					polypeptide-containing ring of GroEL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_30_21251_s_20	10409682	(ii) Bind-ing of ATP to the polypeptide-containing ring of GroEL permits the binding of GroES to that ring accompanying the release of polypeptide into an enclosed cage, defined by the GroEL cavity and the dome of GroES, in which folding to the native state can proceed with aggregation being avoided ( 6,  8-13).	bind
17714	3	5638	6	10	NULL	NULL	NULL	statement 1	Process		permits					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_30_21251_s_20	10409682	(ii) Bind-ing of ATP to the polypeptide-containing ring of GroEL permits the binding of GroES to that ring accompanying the release of polypeptide into an enclosed cage, defined by the GroEL cavity and the dome of GroES, in which folding to the native state can proceed with aggregation being avoided ( 6,  8-13).	bind
17068	1	5638	7	10	NULL	NULL	NULL	ATP	Chemical		bind					polypeptide-containing ring GroEL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_30_21251_s_20	10409682	(ii) Bind-ing of ATP to the polypeptide-containing ring of GroEL permits the binding of GroES to that ring accompanying the release of polypeptide into an enclosed cage, defined by the GroEL cavity and the dome of GroES, in which folding to the native state can proceed with aggregation being avoided ( 6,  8-13).	bind
17071	2	5638	7	10	NULL	NULL	NULL	GroES	GP		bind					polypeptide-containing ring GroEL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_30_21251_s_20	10409682	(ii) Bind-ing of ATP to the polypeptide-containing ring of GroEL permits the binding of GroES to that ring accompanying the release of polypeptide into an enclosed cage, defined by the GroEL cavity and the dome of GroES, in which folding to the native state can proceed with aggregation being avoided ( 6,  8-13).	bind
17072	3	5638	7	10	NULL	NULL	NULL	statement 1	Process		permits					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_30_21251_s_20	10409682	(ii) Bind-ing of ATP to the polypeptide-containing ring of GroEL permits the binding of GroES to that ring accompanying the release of polypeptide into an enclosed cage, defined by the GroEL cavity and the dome of GroES, in which folding to the native state can proceed with aggregation being avoided ( 6,  8-13).	bind
17733	1	5639	6	10	NULL	NULL	NULL	bacteria	Organism		bind					Eap-coated surface	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_6_2933_s_197	12010982	(ii) Binding of bacteria to Eap-coated surface.	bind
17089	1	5639	7	10	NULL	NULL	NULL	bacteria	Organism		bind					Eap-coated surface	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_6_2933_s_197	12010982	(ii) Binding of bacteria to Eap-coated surface.	bind
17734	1	5640	6	10	NULL	NULL	NULL	PGN	GP		bind					CD14	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8680_s_251	9535844	(ii) Binding of PGN to CD14 and the inhibitory capacity of PGN for CD14 binding to PGN and LPS are lost when the PGN preparations are digested with PGN-lytic enzymes (lysostaphin, muramidase SG, and lysozyme) but are not affected by digestion with other enzymes (heparinase, RNase, DNase, and trypsin).	bind
17735	2	5640	6	10	NULL	NULL	NULL	CD14	GP		bind					LPS	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8680_s_251	9535844	(ii) Binding of PGN to CD14 and the inhibitory capacity of PGN for CD14 binding to PGN and LPS are lost when the PGN preparations are digested with PGN-lytic enzymes (lysostaphin, muramidase SG, and lysozyme) but are not affected by digestion with other enzymes (heparinase, RNase, DNase, and trypsin).	bind
17736	3	5640	6	10	NULL	NULL	NULL	PGN	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8680_s_251	9535844	(ii) Binding of PGN to CD14 and the inhibitory capacity of PGN for CD14 binding to PGN and LPS are lost when the PGN preparations are digested with PGN-lytic enzymes (lysostaphin, muramidase SG, and lysozyme) but are not affected by digestion with other enzymes (heparinase, RNase, DNase, and trypsin).	bind
17737	4	5640	6	10	NULL	NULL	NULL	PGN	GP		inhibits					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8680_s_251	9535844	(ii) Binding of PGN to CD14 and the inhibitory capacity of PGN for CD14 binding to PGN and LPS are lost when the PGN preparations are digested with PGN-lytic enzymes (lysostaphin, muramidase SG, and lysozyme) but are not affected by digestion with other enzymes (heparinase, RNase, DNase, and trypsin).	bind
17738	5	5640	6	10	NULL	NULL	NULL	lysostaphin	GP		is a type of					PGN-lytic enzyme	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8680_s_251	9535844	(ii) Binding of PGN to CD14 and the inhibitory capacity of PGN for CD14 binding to PGN and LPS are lost when the PGN preparations are digested with PGN-lytic enzymes (lysostaphin, muramidase SG, and lysozyme) but are not affected by digestion with other enzymes (heparinase, RNase, DNase, and trypsin).	bind
17739	6	5640	6	10	NULL	NULL	NULL	muramidase SG	GP		is a type of					PGN-lytic enzyme	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8680_s_251	9535844	(ii) Binding of PGN to CD14 and the inhibitory capacity of PGN for CD14 binding to PGN and LPS are lost when the PGN preparations are digested with PGN-lytic enzymes (lysostaphin, muramidase SG, and lysozyme) but are not affected by digestion with other enzymes (heparinase, RNase, DNase, and trypsin).	bind
17740	7	5640	6	10	NULL	NULL	NULL	lysozyme	GP		is a type of					PGN-lytic enzyme	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8680_s_251	9535844	(ii) Binding of PGN to CD14 and the inhibitory capacity of PGN for CD14 binding to PGN and LPS are lost when the PGN preparations are digested with PGN-lytic enzymes (lysostaphin, muramidase SG, and lysozyme) but are not affected by digestion with other enzymes (heparinase, RNase, DNase, and trypsin).	bind
17741	8	5640	6	10	NULL	NULL	NULL	statement 5	Process		disrupts					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8680_s_251	9535844	(ii) Binding of PGN to CD14 and the inhibitory capacity of PGN for CD14 binding to PGN and LPS are lost when the PGN preparations are digested with PGN-lytic enzymes (lysostaphin, muramidase SG, and lysozyme) but are not affected by digestion with other enzymes (heparinase, RNase, DNase, and trypsin).	bind
17742	9	5640	6	10	NULL	NULL	NULL	statement 5	Process		disrupts					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8680_s_251	9535844	(ii) Binding of PGN to CD14 and the inhibitory capacity of PGN for CD14 binding to PGN and LPS are lost when the PGN preparations are digested with PGN-lytic enzymes (lysostaphin, muramidase SG, and lysozyme) but are not affected by digestion with other enzymes (heparinase, RNase, DNase, and trypsin).	bind
17743	10	5640	6	10	NULL	NULL	NULL	statement 6	Process		disrupts					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8680_s_251	9535844	(ii) Binding of PGN to CD14 and the inhibitory capacity of PGN for CD14 binding to PGN and LPS are lost when the PGN preparations are digested with PGN-lytic enzymes (lysostaphin, muramidase SG, and lysozyme) but are not affected by digestion with other enzymes (heparinase, RNase, DNase, and trypsin).	bind
17744	11	5640	6	10	NULL	NULL	NULL	statement 6	Process		disrupts					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8680_s_251	9535844	(ii) Binding of PGN to CD14 and the inhibitory capacity of PGN for CD14 binding to PGN and LPS are lost when the PGN preparations are digested with PGN-lytic enzymes (lysostaphin, muramidase SG, and lysozyme) but are not affected by digestion with other enzymes (heparinase, RNase, DNase, and trypsin).	bind
17745	12	5640	6	10	NULL	NULL	NULL	statement 7	Process		disrupts					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8680_s_251	9535844	(ii) Binding of PGN to CD14 and the inhibitory capacity of PGN for CD14 binding to PGN and LPS are lost when the PGN preparations are digested with PGN-lytic enzymes (lysostaphin, muramidase SG, and lysozyme) but are not affected by digestion with other enzymes (heparinase, RNase, DNase, and trypsin).	bind
17746	13	5640	6	10	NULL	NULL	NULL	statement 7	Process		disrupts					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8680_s_251	9535844	(ii) Binding of PGN to CD14 and the inhibitory capacity of PGN for CD14 binding to PGN and LPS are lost when the PGN preparations are digested with PGN-lytic enzymes (lysostaphin, muramidase SG, and lysozyme) but are not affected by digestion with other enzymes (heparinase, RNase, DNase, and trypsin).	bind
17090	1	5640	7	10	NULL	NULL	NULL	PGN	GP		bind					CD14	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8680_s_251	9535844	(ii) Binding of PGN to CD14 and the inhibitory capacity of PGN for CD14 binding to PGN and LPS are lost when the PGN preparations are digested with PGN-lytic enzymes (lysostaphin, muramidase SG, and lysozyme) but are not affected by digestion with other enzymes (heparinase, RNase, DNase, and trypsin).	bind
17091	2	5640	7	10	NULL	NULL	NULL	LPS	Chemical		bind					CD14	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8680_s_251	9535844	(ii) Binding of PGN to CD14 and the inhibitory capacity of PGN for CD14 binding to PGN and LPS are lost when the PGN preparations are digested with PGN-lytic enzymes (lysostaphin, muramidase SG, and lysozyme) but are not affected by digestion with other enzymes (heparinase, RNase, DNase, and trypsin).	bind
17092	3	5640	7	10	NULL	NULL	NULL	PGN	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8680_s_251	9535844	(ii) Binding of PGN to CD14 and the inhibitory capacity of PGN for CD14 binding to PGN and LPS are lost when the PGN preparations are digested with PGN-lytic enzymes (lysostaphin, muramidase SG, and lysozyme) but are not affected by digestion with other enzymes (heparinase, RNase, DNase, and trypsin).	bind
17093	4	5640	7	10	NULL	NULL	NULL	PGN	GP		inhibits					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8680_s_251	9535844	(ii) Binding of PGN to CD14 and the inhibitory capacity of PGN for CD14 binding to PGN and LPS are lost when the PGN preparations are digested with PGN-lytic enzymes (lysostaphin, muramidase SG, and lysozyme) but are not affected by digestion with other enzymes (heparinase, RNase, DNase, and trypsin).	bind
17094	5	5640	7	10	NULL	NULL	NULL	lysostaphin	GP		is a type of					PGN-lytic enzymes	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8680_s_251	9535844	(ii) Binding of PGN to CD14 and the inhibitory capacity of PGN for CD14 binding to PGN and LPS are lost when the PGN preparations are digested with PGN-lytic enzymes (lysostaphin, muramidase SG, and lysozyme) but are not affected by digestion with other enzymes (heparinase, RNase, DNase, and trypsin).	bind
17095	6	5640	7	10	NULL	NULL	NULL	muramidase SG	GP		is a type of					PGN-lytic enzymes	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8680_s_251	9535844	(ii) Binding of PGN to CD14 and the inhibitory capacity of PGN for CD14 binding to PGN and LPS are lost when the PGN preparations are digested with PGN-lytic enzymes (lysostaphin, muramidase SG, and lysozyme) but are not affected by digestion with other enzymes (heparinase, RNase, DNase, and trypsin).	bind
17096	7	5640	7	10	NULL	NULL	NULL	lysozyme	GP		is a type of					PGN-lytic enzymes	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8680_s_251	9535844	(ii) Binding of PGN to CD14 and the inhibitory capacity of PGN for CD14 binding to PGN and LPS are lost when the PGN preparations are digested with PGN-lytic enzymes (lysostaphin, muramidase SG, and lysozyme) but are not affected by digestion with other enzymes (heparinase, RNase, DNase, and trypsin).	bind
17097	8	5640	7	10	NULL	NULL	NULL	statement 5	Process		disrupts					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8680_s_251	9535844	(ii) Binding of PGN to CD14 and the inhibitory capacity of PGN for CD14 binding to PGN and LPS are lost when the PGN preparations are digested with PGN-lytic enzymes (lysostaphin, muramidase SG, and lysozyme) but are not affected by digestion with other enzymes (heparinase, RNase, DNase, and trypsin).	bind
17098	9	5640	7	10	NULL	NULL	NULL	statement 5	Process		disrupts					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8680_s_251	9535844	(ii) Binding of PGN to CD14 and the inhibitory capacity of PGN for CD14 binding to PGN and LPS are lost when the PGN preparations are digested with PGN-lytic enzymes (lysostaphin, muramidase SG, and lysozyme) but are not affected by digestion with other enzymes (heparinase, RNase, DNase, and trypsin).	bind
17099	10	5640	7	10	NULL	NULL	NULL	statement 6	Process		disrupts					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8680_s_251	9535844	(ii) Binding of PGN to CD14 and the inhibitory capacity of PGN for CD14 binding to PGN and LPS are lost when the PGN preparations are digested with PGN-lytic enzymes (lysostaphin, muramidase SG, and lysozyme) but are not affected by digestion with other enzymes (heparinase, RNase, DNase, and trypsin).	bind
45847	11	5640	7	10	NULL	NULL	NULL	statement 6	Process		disrupts					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8680_s_251	9535844	(ii) Binding of PGN to CD14 and the inhibitory capacity of PGN for CD14 binding to PGN and LPS are lost when the PGN preparations are digested with PGN-lytic enzymes (lysostaphin, muramidase SG, and lysozyme) but are not affected by digestion with other enzymes (heparinase, RNase, DNase, and trypsin).	bind
45848	12	5640	7	10	NULL	NULL	NULL	statement 7	Process		disrupts					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8680_s_251	9535844	(ii) Binding of PGN to CD14 and the inhibitory capacity of PGN for CD14 binding to PGN and LPS are lost when the PGN preparations are digested with PGN-lytic enzymes (lysostaphin, muramidase SG, and lysozyme) but are not affected by digestion with other enzymes (heparinase, RNase, DNase, and trypsin).	bind
45849	13	5640	7	10	NULL	NULL	NULL	statement 7	Process		disrupts					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8680_s_251	9535844	(ii) Binding of PGN to CD14 and the inhibitory capacity of PGN for CD14 binding to PGN and LPS are lost when the PGN preparations are digested with PGN-lytic enzymes (lysostaphin, muramidase SG, and lysozyme) but are not affected by digestion with other enzymes (heparinase, RNase, DNase, and trypsin).	bind
17747	1	5641	6	10	NULL	NULL	NULL	Raf	GP		bind					Ras	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4623_s_312	10373511	(ii) Binding of Raf to Ras does not change the intrinsic GTPase activity of Ras (50% conversion of GTP to GDP in about 30 min) ( 10) or slightly enhances it ( 40).	bind
17748	2	5641	6	10	NULL	NULL	NULL	Ras	GP		activates					GTPase	GP	intrinsic			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4623_s_312	10373511	(ii) Binding of Raf to Ras does not change the intrinsic GTPase activity of Ras (50% conversion of GTP to GDP in about 30 min) ( 10) or slightly enhances it ( 40).	bind
17749	3	5641	6	10	NULL	NULL	NULL	statement 1	Process		does not change					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4623_s_312	10373511	(ii) Binding of Raf to Ras does not change the intrinsic GTPase activity of Ras (50% conversion of GTP to GDP in about 30 min) ( 10) or slightly enhances it ( 40).	bind
20310	4	5641	6	10	NULL	NULL	NULL	statement 1	Process		slightly enhances					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4623_s_312	10373511	(ii) Binding of Raf to Ras does not change the intrinsic GTPase activity of Ras (50% conversion of GTP to GDP in about 30 min) ( 10) or slightly enhances it ( 40).	bind
20311	5	5641	6	10	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4623_s_312	10373511	(ii) Binding of Raf to Ras does not change the intrinsic GTPase activity of Ras (50% conversion of GTP to GDP in about 30 min) ( 10) or slightly enhances it ( 40).	bind
17100	1	5641	7	10	NULL	NULL	NULL	Raf	GP		bind					Ras	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4623_s_312	10373511	(ii) Binding of Raf to Ras does not change the intrinsic GTPase activity of Ras (50% conversion of GTP to GDP in about 30 min) ( 10) or slightly enhances it ( 40).	bind
17101	2	5641	7	10	NULL	NULL	NULL	statement 1	GP		does not change					Ras	GP	intrinsic GTPase activity of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4623_s_312	10373511	(ii) Binding of Raf to Ras does not change the intrinsic GTPase activity of Ras (50% conversion of GTP to GDP in about 30 min) ( 10) or slightly enhances it ( 40).	bind
17102	3	5641	7	10	NULL	NULL	NULL	statement 1	Process		enhance		slightly			Ras	GP	intrinsic GTPase activity of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4623_s_312	10373511	(ii) Binding of Raf to Ras does not change the intrinsic GTPase activity of Ras (50% conversion of GTP to GDP in about 30 min) ( 10) or slightly enhances it ( 40).	bind
17103	4	5641	7	10	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4623_s_312	10373511	(ii) Binding of Raf to Ras does not change the intrinsic GTPase activity of Ras (50% conversion of GTP to GDP in about 30 min) ( 10) or slightly enhances it ( 40).	bind
17750	1	5642	6	10	NULL	NULL	NULL	surface proteins	GP		bind					choline 	Chemical	containing teichoic acids			NULL	Streptococcus pneumoniae	NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1694_1_269_s_10	15546671	(ii) Binding of surface proteins to choline containing teichoic acids (in  Streptococcus pneumoniae) [  9].	bind
17104	1	5642	7	10	NULL	NULL	NULL	surface proteins	GP		bind					choline	Chemical	containing teichoic acids			NULL	Streptococcus pneumoniae	NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1694_1_269_s_10	15546671	(ii) Binding of surface proteins to choline containing teichoic acids (in  Streptococcus pneumoniae) [  9].	bind
17751	1	5643	6	10	NULL	NULL	NULL	Wzt	GP		bind					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_7_4458_s_91	11401986	(ii) Binding of Wzt to ATP.	bind
17105	1	5643	7	10	NULL	NULL	NULL	Wzt	GP		bind					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_7_4458_s_91	11401986	(ii) Binding of Wzt to ATP.	bind
17752	1	5645	6	10	NULL	NULL	NULL	ghrelin	GP		bind					GHSR-1a	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_6_1029_s_151	12486113	(ii) Both ghrelin and its deacylated form, des-acyl ghrelin, recognize a common high affinity binding site, although only ghrelin and not des-acyl ghrelin bind to GHSR-1a ( Kojima et al., 1999).	bind
17753	2	5645	6	10	NULL	NULL	NULL	des-acyl ghrelin	GP		does not bind					GHSR-1a	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_6_1029_s_151	12486113	(ii) Both ghrelin and its deacylated form, des-acyl ghrelin, recognize a common high affinity binding site, although only ghrelin and not des-acyl ghrelin bind to GHSR-1a ( Kojima et al., 1999).	bind
45630	3	5645	6	10	NULL	NULL	NULL	des-acyl ghrelin	GP		is deacylated form of					ghrelin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_6_1029_s_151	12486113	(ii) Both ghrelin and its deacylated form, des-acyl ghrelin, recognize a common high affinity binding site, although only ghrelin and not des-acyl ghrelin bind to GHSR-1a ( Kojima et al., 1999).	bind
17107	1	5645	7	10	NULL	NULL	NULL	ghrelin	GP		bind					GHSR-1a	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_6_1029_s_151	12486113	(ii) Both ghrelin and its deacylated form, des-acyl ghrelin, recognize a common high affinity binding site, although only ghrelin and not des-acyl ghrelin bind to GHSR-1a ( Kojima et al., 1999).	bind
17108	2	5645	7	10	NULL	NULL	NULL	des-acyl ghrelin	GP		does not bind					GHSR-1a	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_6_1029_s_151	12486113	(ii) Both ghrelin and its deacylated form, des-acyl ghrelin, recognize a common high affinity binding site, although only ghrelin and not des-acyl ghrelin bind to GHSR-1a ( Kojima et al., 1999).	bind
17109	3	5645	7	10	NULL	NULL	NULL	des-acyl ghrelin	GP		is deacylated form of					ghrelin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_6_1029_s_151	12486113	(ii) Both ghrelin and its deacylated form, des-acyl ghrelin, recognize a common high affinity binding site, although only ghrelin and not des-acyl ghrelin bind to GHSR-1a ( Kojima et al., 1999).	bind
17754	1	5646	6	10	NULL	NULL	NULL	E2	GP		bind					ER	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_4_1978_s_274	16314411	(ii) Ca2+/calmodulin stimulates E2 binding to the ER ( ).	bind
17755	2	5646	6	10	NULL	NULL	NULL	Ca2+	Chemical		stimulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_4_1978_s_274	16314411	(ii) Ca2+/calmodulin stimulates E2 binding to the ER ( ).	bind
67377	3	5646	6	10	NULL	0	NULL	calmodulin	GP		stimulates					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_4_1978_s_274	16314411	(ii) Ca2+/calmodulin stimulates E2 binding to the ER ( ).	bind
17110	1	5646	7	10	NULL	NULL	NULL	E2	GP		bind					ER	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_4_1978_s_274	16314411	(ii) Ca2+/calmodulin stimulates E2 binding to the ER ( ).	bind
17111	2	5646	7	10	NULL	NULL	NULL	Ca2+	Chemical		stimulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_4_1978_s_274	16314411	(ii) Ca2+/calmodulin stimulates E2 binding to the ER ( ).	bind
67378	3	5646	7	10	NULL	0	NULL	calmodulin	GP		stimulates					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_4_1978_s_274	16314411	(ii) Ca2+/calmodulin stimulates E2 binding to the ER ( ).	bind
17756	1	5649	6	10	NULL	NULL	NULL	statins	gP		bind					LFA-1	GP				NULL	antigen presenting cells	NULL	NULL	NULL	NULL	gw70_atherosclerosis_175_1_83_s_12	15186950	(ii) Certain statins bind to the adhesion molecule leucocyte function antigen-1  (LFA-1) on antigen-presenting cells and therefore block the interaction with T cells  expressing the counter-receptor intercellular adhesion molecule-1 (ICAM-1) [  12].	bind
17757	2	5649	6	10	NULL	NULL	NULL	LFA-1	GP		is					leucocyte function antigen-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_atherosclerosis_175_1_83_s_12	15186950	(ii) Certain statins bind to the adhesion molecule leucocyte function antigen-1  (LFA-1) on antigen-presenting cells and therefore block the interaction with T cells  expressing the counter-receptor intercellular adhesion molecule-1 (ICAM-1) [  12].	bind
17758	3	5649	6	10	NULL	NULL	NULL	ICAM-1	GP		is					intercellular adhesion molecule-1 	GP				NULL		NULL	NULL	NULL	NULL	gw70_atherosclerosis_175_1_83_s_12	15186950	(ii) Certain statins bind to the adhesion molecule leucocyte function antigen-1  (LFA-1) on antigen-presenting cells and therefore block the interaction with T cells  expressing the counter-receptor intercellular adhesion molecule-1 (ICAM-1) [  12].	bind
17759	4	5649	6	10	NULL	NULL	NULL	T cells	Cell		express					ICAM-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_atherosclerosis_175_1_83_s_12	15186950	(ii) Certain statins bind to the adhesion molecule leucocyte function antigen-1  (LFA-1) on antigen-presenting cells and therefore block the interaction with T cells  expressing the counter-receptor intercellular adhesion molecule-1 (ICAM-1) [  12].	bind
17760	5	5649	6	10	NULL	NULL	NULL	statement 1	Process		block					statement 4	Process	 interaction with			NULL		NULL	NULL	NULL	NULL	gw70_atherosclerosis_175_1_83_s_12	15186950	(ii) Certain statins bind to the adhesion molecule leucocyte function antigen-1  (LFA-1) on antigen-presenting cells and therefore block the interaction with T cells  expressing the counter-receptor intercellular adhesion molecule-1 (ICAM-1) [  12].	bind
45631	6	5649	6	10	NULL	NULL	NULL	LFA-1	GP		is a type of					adhesion molecule	GP				NULL		NULL	NULL	NULL	NULL	gw70_atherosclerosis_175_1_83_s_12	15186950	(ii) Certain statins bind to the adhesion molecule leucocyte function antigen-1  (LFA-1) on antigen-presenting cells and therefore block the interaction with T cells  expressing the counter-receptor intercellular adhesion molecule-1 (ICAM-1) [  12].	bind
45632	7	5649	6	10	NULL	NULL	NULL	ICAM-1	GP		is a type of					counter-receptor molecule	GP				NULL		NULL	NULL	NULL	NULL	gw70_atherosclerosis_175_1_83_s_12	15186950	(ii) Certain statins bind to the adhesion molecule leucocyte function antigen-1  (LFA-1) on antigen-presenting cells and therefore block the interaction with T cells  expressing the counter-receptor intercellular adhesion molecule-1 (ICAM-1) [  12].	bind
17112	1	5649	7	10	NULL	NULL	NULL	statins	GP		bind					LFA-1	GP				NULL	antigen-presenting cells	NULL	NULL	NULL	NULL	gw70_atherosclerosis_175_1_83_s_12	15186950	(ii) Certain statins bind to the adhesion molecule leucocyte function antigen-1  (LFA-1) on antigen-presenting cells and therefore block the interaction with T cells  expressing the counter-receptor intercellular adhesion molecule-1 (ICAM-1) [  12].	bind
17113	2	5649	7	10	NULL	NULL	NULL	antigen-presenting cells	Cell		bind					T cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_atherosclerosis_175_1_83_s_12	15186950	(ii) Certain statins bind to the adhesion molecule leucocyte function antigen-1  (LFA-1) on antigen-presenting cells and therefore block the interaction with T cells  expressing the counter-receptor intercellular adhesion molecule-1 (ICAM-1) [  12].	bind
17114	3	5649	7	10	NULL	NULL	NULL	T cells	Cell		express					ICAM-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_atherosclerosis_175_1_83_s_12	15186950	(ii) Certain statins bind to the adhesion molecule leucocyte function antigen-1  (LFA-1) on antigen-presenting cells and therefore block the interaction with T cells  expressing the counter-receptor intercellular adhesion molecule-1 (ICAM-1) [  12].	bind
17115	4	5649	7	10	NULL	NULL	NULL	statement 1	Process		blocks					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_atherosclerosis_175_1_83_s_12	15186950	(ii) Certain statins bind to the adhesion molecule leucocyte function antigen-1  (LFA-1) on antigen-presenting cells and therefore block the interaction with T cells  expressing the counter-receptor intercellular adhesion molecule-1 (ICAM-1) [  12].	bind
17117	6	5649	7	10	NULL	NULL	NULL	LFA-1	GP		is					leucocyte function antigen-1 	GP				NULL		NULL	NULL	NULL	NULL	gw70_atherosclerosis_175_1_83_s_12	15186950	(ii) Certain statins bind to the adhesion molecule leucocyte function antigen-1  (LFA-1) on antigen-presenting cells and therefore block the interaction with T cells  expressing the counter-receptor intercellular adhesion molecule-1 (ICAM-1) [  12].	bind
17118	7	5649	7	10	NULL	NULL	NULL	ICAM-1	GP		is					intercellular adhesion molecule-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_atherosclerosis_175_1_83_s_12	15186950	(ii) Certain statins bind to the adhesion molecule leucocyte function antigen-1  (LFA-1) on antigen-presenting cells and therefore block the interaction with T cells  expressing the counter-receptor intercellular adhesion molecule-1 (ICAM-1) [  12].	bind
17119	8	5649	7	10	NULL	NULL	NULL	LFA-1	GP		is a type of					adhesion molecule	GP				NULL		NULL	NULL	NULL	NULL	gw70_atherosclerosis_175_1_83_s_12	15186950	(ii) Certain statins bind to the adhesion molecule leucocyte function antigen-1  (LFA-1) on antigen-presenting cells and therefore block the interaction with T cells  expressing the counter-receptor intercellular adhesion molecule-1 (ICAM-1) [  12].	bind
17120	9	5649	7	10	NULL	NULL	NULL	ICAM-1	GP		is a type of					counter-receptor molecule	GP				NULL		NULL	NULL	NULL	NULL	gw70_atherosclerosis_175_1_83_s_12	15186950	(ii) Certain statins bind to the adhesion molecule leucocyte function antigen-1  (LFA-1) on antigen-presenting cells and therefore block the interaction with T cells  expressing the counter-receptor intercellular adhesion molecule-1 (ICAM-1) [  12].	bind
17761	1	5650	6	10	NULL	NULL	NULL	CTCF	GP		does not bind					ICR	GP			insulator sites	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_11_4791_s_234	15143173	(ii) CTCF binds to other sequences in the ICR -- aside from the insulator sites -- to inhibit methylation.	bind
17762	2	5650	6	10	NULL	NULL	NULL	CTCF	GP		bind					ICR	GP			other sequences	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_11_4791_s_234	15143173	(ii) CTCF binds to other sequences in the ICR -- aside from the insulator sites -- to inhibit methylation.	bind
17763	3	5650	6	10	NULL	NULL	NULL	statement 2	Process		inhibits					methylation	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_11_4791_s_234	15143173	(ii) CTCF binds to other sequences in the ICR -- aside from the insulator sites -- to inhibit methylation.	bind
17121	1	5650	7	10	NULL	NULL	NULL	CTCF	GP		binds					 ICR	GP			sequences	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_11_4791_s_234	15143173	(ii) CTCF binds to other sequences in the ICR -- aside from the insulator sites -- to inhibit methylation.	bind
17122	2	5650	7	10	NULL	NULL	NULL	CTCF	GP		does not bind					ICR	GP			insulator sites	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_11_4791_s_234	15143173	(ii) CTCF binds to other sequences in the ICR -- aside from the insulator sites -- to inhibit methylation.	bind
17123	3	5650	7	10	NULL	NULL	NULL	statement 1	Process		inhibits					methylation	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_11_4791_s_234	15143173	(ii) CTCF binds to other sequences in the ICR -- aside from the insulator sites -- to inhibit methylation.	bind
17764	1	5651	6	10	NULL	NULL	NULL	Vn	GP	denatured	bind		dose dependently			glycoprotein IIb/IIa	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_21_13705_s_7	9153222	(ii) Denatured Vn binds to both glycoprotein IIb/IIa and alphavbeta3 in a dose-dependent manner.	bind
17765	2	5651	6	10	NULL	NULL	NULL	Vn	GP	denatured	bind		dose dependently			alphavbeta3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_21_13705_s_7	9153222	(ii) Denatured Vn binds to both glycoprotein IIb/IIa and alphavbeta3 in a dose-dependent manner.	bind
17124	1	5651	7	10	NULL	NULL	NULL	Vn 	GP	denatured	bind		dose-dependently			glycoprotein IIb/IIa	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_21_13705_s_7	9153222	(ii) Denatured Vn binds to both glycoprotein IIb/IIa and alphavbeta3 in a dose-dependent manner.	bind
17125	2	5651	7	10	NULL	NULL	NULL	Vn	GP	denatured	bind		dose-dependently			alphavbeta3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_21_13705_s_7	9153222	(ii) Denatured Vn binds to both glycoprotein IIb/IIa and alphavbeta3 in a dose-dependent manner.	bind
17766	1	5652	6	10	NULL	NULL	NULL	DicB	GP 		have affinity for a					septal ring factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_11_2951_s_264	12003935	(ii) DicB itself might have affinity for a septal ring factor and recruit MinC. (iii) The binding of DicB to MinC might create a site on the heteromeric complex with a high affinity for a septal ring-associated target.	bind
17767	2	5652	6	10	NULL	NULL	NULL	DicB	GP		recruit					MinC	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_11_2951_s_264	12003935	(ii) DicB itself might have affinity for a septal ring factor and recruit MinC. (iii) The binding of DicB to MinC might create a site on the heteromeric complex with a high affinity for a septal ring-associated target.	bind
17768	3	5652	6	10	NULL	NULL	NULL	DicB	GP		bind					MinC	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_11_2951_s_264	12003935	(ii) DicB itself might have affinity for a septal ring factor and recruit MinC. (iii) The binding of DicB to MinC might create a site on the heteromeric complex with a high affinity for a septal ring-associated target.	bind
17769	4	5652	6	10	NULL	NULL	NULL	statement 3	Process		create		may			heteromeric complex	GP		site		NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_11_2951_s_264	12003935	(ii) DicB itself might have affinity for a septal ring factor and recruit MinC. (iii) The binding of DicB to MinC might create a site on the heteromeric complex with a high affinity for a septal ring-associated target.	bind
17770	5	5652	6	10	NULL	NULL	NULL	heteromeric complex	GP		has high affinity for					septal ring-associated target	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_11_2951_s_264	12003935	(ii) DicB itself might have affinity for a septal ring factor and recruit MinC. (iii) The binding of DicB to MinC might create a site on the heteromeric complex with a high affinity for a septal ring-associated target.	bind
17128	1	5652	7	10	NULL	NULL	NULL	DicB	GP		 has affinity for					septal ring factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_11_2951_s_264	12003935	(ii) DicB itself might have affinity for a septal ring factor and recruit MinC. (iii) The binding of DicB to MinC might create a site on the heteromeric complex with a high affinity for a septal ring-associated target.	bind
17129	2	5652	7	10	NULL	NULL	NULL	DicB	GP		recruit					MinC	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_11_2951_s_264	12003935	(ii) DicB itself might have affinity for a septal ring factor and recruit MinC. (iii) The binding of DicB to MinC might create a site on the heteromeric complex with a high affinity for a septal ring-associated target.	bind
17130	4	5652	7	10	NULL	NULL	NULL	statement 3	Process		create					heteromeric complex	GP	a site on the			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_11_2951_s_264	12003935	(ii) DicB itself might have affinity for a septal ring factor and recruit MinC. (iii) The binding of DicB to MinC might create a site on the heteromeric complex with a high affinity for a septal ring-associated target.	bind
17131	5	5652	7	10	NULL	NULL	NULL	heteromeric complex	GP		high affinity for					septal ring-associated target	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_11_2951_s_264	12003935	(ii) DicB itself might have affinity for a septal ring factor and recruit MinC. (iii) The binding of DicB to MinC might create a site on the heteromeric complex with a high affinity for a septal ring-associated target.	bind
45850	3	5652	7	10	NULL	NULL	NULL	DicB	GP		bind					MinC	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_11_2951_s_264	12003935	(ii) DicB itself might have affinity for a septal ring factor and recruit MinC. (iii) The binding of DicB to MinC might create a site on the heteromeric complex with a high affinity for a septal ring-associated target.	bind
17358	1	5653	7	10	NULL	NULL	NULL	GPVI	GP		bind					Fc Rgamma	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_17_15441_s_214	12594225	(ii) Does GPVI interact with Fc Rgamma, calmodulin, and Lyn through discrete protein domains or does the receptor interact with these proteins in an interdependent fashion that requires formation of a complex in which some or all must be present?	bind
17359	2	5653	7	10	NULL	NULL	NULL	GPVI	GP		bind					calmodulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_17_15441_s_214	12594225	(ii) Does GPVI interact with Fc Rgamma, calmodulin, and Lyn through discrete protein domains or does the receptor interact with these proteins in an interdependent fashion that requires formation of a complex in which some or all must be present?	bind
17360	3	5653	7	10	NULL	NULL	NULL	GPVI	GP		bind					Lyn	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_17_15441_s_214	12594225	(ii) Does GPVI interact with Fc Rgamma, calmodulin, and Lyn through discrete protein domains or does the receptor interact with these proteins in an interdependent fashion that requires formation of a complex in which some or all must be present?	bind
17778	1	5654	6	10	NULL	NULL	NULL	G6P	GP		bind		strongly;;anti-cooperatively			HKI	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_44_31155_s_32	10531306	(ii) G6P binding to HKI must be strongly anti-cooperative.	bind
17132	1	5654	7	10	NULL	NULL	NULL	G6P	GP		bind		strongly;;anti-cooperatively			HKI 	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_44_31155_s_32	10531306	(ii) G6P binding to HKI must be strongly anti-cooperative.	bind
17779	1	5655	6	10	NULL	NULL	NULL	HSP90	GP		bind					eNOS	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_11_9339_s_191	12519764	(ii) HSP90 binding to eNOS increases when the quantity of CaM bound to eNOS remains constant (Fig.  5), and this results in a further increase in eNOS activity (from 139% to 254% of basal eNOS activity at 12 and 45 nM HSP90, respectively; Fig.  2).	bind
17780	2	5655	6	10	NULL	NULL	NULL	CaM	GP		bind					eNOS	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_11_9339_s_191	12519764	(ii) HSP90 binding to eNOS increases when the quantity of CaM bound to eNOS remains constant (Fig.  5), and this results in a further increase in eNOS activity (from 139% to 254% of basal eNOS activity at 12 and 45 nM HSP90, respectively; Fig.  2).	bind
17134	1	5655	7	10	NULL	NULL	NULL	HSP90	GP		bind					eNOS	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_11_9339_s_191	12519764	(ii) HSP90 binding to eNOS increases when the quantity of CaM bound to eNOS remains constant (Fig.  5), and this results in a further increase in eNOS activity (from 139% to 254% of basal eNOS activity at 12 and 45 nM HSP90, respectively; Fig.  2).	bind
17135	2	5655	7	10	NULL	NULL	NULL	CaM	GP		bind					eNOS	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_11_9339_s_191	12519764	(ii) HSP90 binding to eNOS increases when the quantity of CaM bound to eNOS remains constant (Fig.  5), and this results in a further increase in eNOS activity (from 139% to 254% of basal eNOS activity at 12 and 45 nM HSP90, respectively; Fig.  2).	bind
17906	1	5656	6	10	NULL	NULL	NULL	Sm proteins	GP		assemble onto					oligonucleotide	NucleicAcid	consensus		Sm binding site 	NULL	Xenopus oocytes	NULL	NULL	NULL	NULL	gw60_embo_20_19_5470_s_206	11574479	(ii) In a study of the assembly of U7 snRNPs in  Xenopus oocytes ( Stefanovic  et al., 1995), we have previously shown that the Sm B and G proteins could be cross-linked to the Sm binding site of U7 snRNA to similar positions as have recently been characterized for Sm proteins assembled onto a consensus Sm binding site oligonucleotide ( Urlaub  et al., 2001).	bind
17907	2	5656	6	10	NULL	NULL	NULL	Sm B proteins	GP		cross link		may			U7 snRNA	NucleicAcid		Sm binding site		NULL	Xenopus oocytes	NULL	NULL	NULL	NULL	gw60_embo_20_19_5470_s_206	11574479	(ii) In a study of the assembly of U7 snRNPs in  Xenopus oocytes ( Stefanovic  et al., 1995), we have previously shown that the Sm B and G proteins could be cross-linked to the Sm binding site of U7 snRNA to similar positions as have recently been characterized for Sm proteins assembled onto a consensus Sm binding site oligonucleotide ( Urlaub  et al., 2001).	bind
17908	3	5656	6	10	NULL	NULL	NULL	Sm G protein	GP		cross link		may			U7 snRNA	NucleicAcid		Sm binding site		NULL	Xenopus oocytes	NULL	NULL	NULL	NULL	gw60_embo_20_19_5470_s_206	11574479	(ii) In a study of the assembly of U7 snRNPs in  Xenopus oocytes ( Stefanovic  et al., 1995), we have previously shown that the Sm B and G proteins could be cross-linked to the Sm binding site of U7 snRNA to similar positions as have recently been characterized for Sm proteins assembled onto a consensus Sm binding site oligonucleotide ( Urlaub  et al., 2001).	bind
17139	1	5656	7	10	NULL	NULL	NULL	Sm B	GP		crosslink to					U7 snRNA	NucleicAcid		Sm binding site 		NULL	 Xenopus oocytes 	NULL	NULL	NULL	NULL	gw60_embo_20_19_5470_s_206	11574479	(ii) In a study of the assembly of U7 snRNPs in  Xenopus oocytes ( Stefanovic  et al., 1995), we have previously shown that the Sm B and G proteins could be cross-linked to the Sm binding site of U7 snRNA to similar positions as have recently been characterized for Sm proteins assembled onto a consensus Sm binding site oligonucleotide ( Urlaub  et al., 2001).	bind
17140	2	5656	7	10	NULL	NULL	NULL	G proteins	GP		crosslink to					U7 snRNA	NucleicAcid		Sm binding site 		NULL	 Xenopus oocytes 	NULL	NULL	NULL	NULL	gw60_embo_20_19_5470_s_206	11574479	(ii) In a study of the assembly of U7 snRNPs in  Xenopus oocytes ( Stefanovic  et al., 1995), we have previously shown that the Sm B and G proteins could be cross-linked to the Sm binding site of U7 snRNA to similar positions as have recently been characterized for Sm proteins assembled onto a consensus Sm binding site oligonucleotide ( Urlaub  et al., 2001).	bind
17141	3	5656	7	10	NULL	NULL	NULL	Sm protein	GP		assemble onto					oligonucleotide	NucleicAcid	consensus		Sm binding site	NULL	 Xenopus oocytes 	NULL	NULL	NULL	NULL	gw60_embo_20_19_5470_s_206	11574479	(ii) In a study of the assembly of U7 snRNPs in  Xenopus oocytes ( Stefanovic  et al., 1995), we have previously shown that the Sm B and G proteins could be cross-linked to the Sm binding site of U7 snRNA to similar positions as have recently been characterized for Sm proteins assembled onto a consensus Sm binding site oligonucleotide ( Urlaub  et al., 2001).	bind
17783	1	5657	6	10	NULL	NULL	NULL	ICP0	GP		bind			RING finger domain		cdc34	GP				NULL	in vitro	NULL	NULL	NULL	NULL	abs-batch0517-0529_proc-natl-acad-sci-u-s-a_98_15_11447293_s_6	11447293	(ii) In an in vitro substrate-independent  ubiquitination system, the RING finger domain encoded by exon 2 of ICP0  binds cdc34, whereas the carboxyl-terminal domain of ICP0 functions as  an E3 ligase independent of the RING finger domain.	bind
17785	2	5657	6	10	NULL	NULL	NULL	ICP0	GP		functions as			carboxyl-terminal domain		E3 ligase	GP				NULL	in vitro	NULL	NULL	NULL	NULL	abs-batch0517-0529_proc-natl-acad-sci-u-s-a_98_15_11447293_s_6	11447293	(ii) In an in vitro substrate-independent  ubiquitination system, the RING finger domain encoded by exon 2 of ICP0  binds cdc34, whereas the carboxyl-terminal domain of ICP0 functions as  an E3 ligase independent of the RING finger domain.	bind
17788	3	5657	6	10	NULL	NULL	NULL	statement 2	Process		is independent of								RING finger domain		NULL	in vitro	NULL	NULL	NULL	NULL	abs-batch0517-0529_proc-natl-acad-sci-u-s-a_98_15_11447293_s_6	11447293	(ii) In an in vitro substrate-independent  ubiquitination system, the RING finger domain encoded by exon 2 of ICP0  binds cdc34, whereas the carboxyl-terminal domain of ICP0 functions as  an E3 ligase independent of the RING finger domain.	bind
20314	4	5657	6	10	NULL	NULL	NULL	ICP0	GP		is encoded by			RING finger domain		ICP0	GP			exon 2	NULL	in vitro	NULL	NULL	NULL	NULL	abs-batch0517-0529_proc-natl-acad-sci-u-s-a_98_15_11447293_s_6	11447293	(ii) In an in vitro substrate-independent  ubiquitination system, the RING finger domain encoded by exon 2 of ICP0  binds cdc34, whereas the carboxyl-terminal domain of ICP0 functions as  an E3 ligase independent of the RING finger domain.	bind
17142	1	5657	7	10	NULL	NULL	NULL	 ICP0	GP		binds			RING finger domain		cdc34	GP				NULL	in vitro	NULL	NULL	NULL	NULL	abs-batch0517-0529_proc-natl-acad-sci-u-s-a_98_15_11447293_s_6	11447293	(ii) In an in vitro substrate-independent  ubiquitination system, the RING finger domain encoded by exon 2 of ICP0  binds cdc34, whereas the carboxyl-terminal domain of ICP0 functions as  an E3 ligase independent of the RING finger domain.	bind
17143	2	5657	7	10	NULL	NULL	NULL	ICP0 	GP		is encoded by			RING finger domain		 ICP0	GP			exon 2	NULL	in vitro	NULL	NULL	NULL	NULL	abs-batch0517-0529_proc-natl-acad-sci-u-s-a_98_15_11447293_s_6	11447293	(ii) In an in vitro substrate-independent  ubiquitination system, the RING finger domain encoded by exon 2 of ICP0  binds cdc34, whereas the carboxyl-terminal domain of ICP0 functions as  an E3 ligase independent of the RING finger domain.	bind
17145	3	5657	7	10	NULL	NULL	NULL	 ICP0	GP		functions as 			 carboxyl-terminal domain		E3 ligase	GP				NULL	in vitro	NULL	NULL	NULL	NULL	abs-batch0517-0529_proc-natl-acad-sci-u-s-a_98_15_11447293_s_6	11447293	(ii) In an in vitro substrate-independent  ubiquitination system, the RING finger domain encoded by exon 2 of ICP0  binds cdc34, whereas the carboxyl-terminal domain of ICP0 functions as  an E3 ligase independent of the RING finger domain.	bind
17146	4	5657	7	10	NULL	NULL	NULL	statement 4	Process		is independent of								RING finger domain		NULL	in vitro	NULL	NULL	NULL	NULL	abs-batch0517-0529_proc-natl-acad-sci-u-s-a_98_15_11447293_s_6	11447293	(ii) In an in vitro substrate-independent  ubiquitination system, the RING finger domain encoded by exon 2 of ICP0  binds cdc34, whereas the carboxyl-terminal domain of ICP0 functions as  an E3 ligase independent of the RING finger domain.	bind
17789	1	5658	6	10	NULL	NULL	NULL	VLDL	Chemical		bind					HSPG-LPL complexes	GP				NULL		NULL	NULL	NULL	NULL	gw60_atherosclerosis_136_2_255_s_156	9543096	(ii) In our experiments we studied binding of VLDL to HSPG-LPL complexes rather than to HSPG or heparin alone, which we consider as more relevant for extrapolation to the in vivo situation.	bind
17147	1	5658	7	10	NULL	NULL	NULL	VLDL	Chemical		bind					HSPG-LPL complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_atherosclerosis_136_2_255_s_156	9543096	(ii) In our experiments we studied binding of VLDL to HSPG-LPL complexes rather than to HSPG or heparin alone, which we consider as more relevant for extrapolation to the in vivo situation.	bind
17790	1	5659	6	10	NULL	NULL	NULL	oral Actinomyces viscosus strains	Organism	rat	bind		preferentially			statherin	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7224_s_6	11705891	(ii) In preferential statherin binding, oral  Actinomyces viscosus strains of rat and hamster origin (and strain 19246 from a human case of actinomycosis) bound statherin preferentially.	bind
17791	2	5659	6	10	NULL	NULL	NULL	oral Actinomyces viscosus strains	Organism	hamster	bind		preferentially			statherin	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7224_s_6	11705891	(ii) In preferential statherin binding, oral  Actinomyces viscosus strains of rat and hamster origin (and strain 19246 from a human case of actinomycosis) bound statherin preferentially.	bind
17792	3	5659	6	10	NULL	NULL	NULL	strain 19246 of actinomycosis	Organism	human	bind		preferentially			statherin	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7224_s_6	11705891	(ii) In preferential statherin binding, oral  Actinomyces viscosus strains of rat and hamster origin (and strain 19246 from a human case of actinomycosis) bound statherin preferentially.	bind
17148	1	5659	7	10	NULL	NULL	NULL	oral Actinomyces viscosus strains 	Organism	rat origin	bind		preferentially			statherin	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7224_s_6	11705891	(ii) In preferential statherin binding, oral  Actinomyces viscosus strains of rat and hamster origin (and strain 19246 from a human case of actinomycosis) bound statherin preferentially.	bind
17149	2	5659	7	10	NULL	NULL	NULL	oral Actinomyces viscosus strains 	Organism	hamster origin	bind		preferentially			statherin	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7224_s_6	11705891	(ii) In preferential statherin binding, oral  Actinomyces viscosus strains of rat and hamster origin (and strain 19246 from a human case of actinomycosis) bound statherin preferentially.	bind
17150	3	5659	7	10	NULL	NULL	NULL	strain 19246	Organism	human	bind		preferentially			statherin	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7224_s_6	11705891	(ii) In preferential statherin binding, oral  Actinomyces viscosus strains of rat and hamster origin (and strain 19246 from a human case of actinomycosis) bound statherin preferentially.	bind
17793	1	5660	6	10	NULL	NULL	NULL	myocyte nuclear factor	GP		bind									PNR element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7243_s_322	9819411	(ii) In the competition assay, although two inverted repeats of the Ets-binding sites were found to be necessary for the myocyte nuclear factor to bind to the PNR element, the HeLa cell nuclear factor could bind effectively to a single Ets-binding site of the palindrome.	bind
17794	2	5660	6	10	NULL	NULL	NULL	HeLa cell nuclear factor	GP		bind		effectively					single		Ets-binding site of the palindrome	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7243_s_322	9819411	(ii) In the competition assay, although two inverted repeats of the Ets-binding sites were found to be necessary for the myocyte nuclear factor to bind to the PNR element, the HeLa cell nuclear factor could bind effectively to a single Ets-binding site of the palindrome.	bind
17795	3	5660	6	10	NULL	NULL	NULL				are necessary for				two inverted repeats of Ets-binding sites	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7243_s_322	9819411	(ii) In the competition assay, although two inverted repeats of the Ets-binding sites were found to be necessary for the myocyte nuclear factor to bind to the PNR element, the HeLa cell nuclear factor could bind effectively to a single Ets-binding site of the palindrome.	bind
17151	1	5660	7	10	NULL	NULL	NULL	myocyte nuclear factor	GP		bind									PNR element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7243_s_322	9819411	(ii) In the competition assay, although two inverted repeats of the Ets-binding sites were found to be necessary for the myocyte nuclear factor to bind to the PNR element, the HeLa cell nuclear factor could bind effectively to a single Ets-binding site of the palindrome.	bind
17152	2	5660	7	10	NULL	NULL	NULL	HeLa cell nuclear factor	GP		bind		effectively					single		Ets-binding site of the palindrome	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7243_s_322	9819411	(ii) In the competition assay, although two inverted repeats of the Ets-binding sites were found to be necessary for the myocyte nuclear factor to bind to the PNR element, the HeLa cell nuclear factor could bind effectively to a single Ets-binding site of the palindrome.	bind
17153	3	5660	7	10	NULL	NULL	NULL				is necessary for				 two inverted repeats of Ets-binding sites	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7243_s_322	9819411	(ii) In the competition assay, although two inverted repeats of the Ets-binding sites were found to be necessary for the myocyte nuclear factor to bind to the PNR element, the HeLa cell nuclear factor could bind effectively to a single Ets-binding site of the palindrome.	bind
17796	1	5661	6	10	NULL	NULL	NULL	ClpA	GP	E.coli	bind					GFP	GP	unfolded			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbacteriol_183_8_2677_s_128	11274130	(ii) In vitro experiments showed that  E. coli ClpA can bind unfolded GFP and that the complex ClpAP can degrade unfolded GFP but not native GFP ( 10).	bind
17797	2	5661	6	10	NULL	NULL	NULL	complex ClpAP	GP		degrade					GFP	GP	unfolded			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbacteriol_183_8_2677_s_128	11274130	(ii) In vitro experiments showed that  E. coli ClpA can bind unfolded GFP and that the complex ClpAP can degrade unfolded GFP but not native GFP ( 10).	bind
17798	3	5661	6	10	NULL	NULL	NULL	complex ClpAP	GP		does not degrade					GFP	GP	native			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbacteriol_183_8_2677_s_128	11274130	(ii) In vitro experiments showed that  E. coli ClpA can bind unfolded GFP and that the complex ClpAP can degrade unfolded GFP but not native GFP ( 10).	bind
17154	1	5661	7	10	NULL	NULL	NULL	ClpA	GP	E. coli	bind					 GFP	GP	unfolded			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbacteriol_183_8_2677_s_128	11274130	(ii) In vitro experiments showed that  E. coli ClpA can bind unfolded GFP and that the complex ClpAP can degrade unfolded GFP but not native GFP ( 10).	bind
17155	2	5661	7	10	NULL	NULL	NULL	ClpA complex	GP		degrade					 GFP	GP	unfolded			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbacteriol_183_8_2677_s_128	11274130	(ii) In vitro experiments showed that  E. coli ClpA can bind unfolded GFP and that the complex ClpAP can degrade unfolded GFP but not native GFP ( 10).	bind
17156	3	5661	7	10	NULL	NULL	NULL	ClpAP complex	GP		does not degrade					GFP	GP	native			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbacteriol_183_8_2677_s_128	11274130	(ii) In vitro experiments showed that  E. coli ClpA can bind unfolded GFP and that the complex ClpAP can degrade unfolded GFP but not native GFP ( 10).	bind
17799	1	5662	6	10	NULL	NULL	NULL	Nrf2/MafK heterodimer	GP	putative	bind									ARE	NULL		NULL	NULL	NULL	NULL	abs-batch0540-0549_free-radic-biol-med_39_11_16274879_s_6	16274879	(ii) Nuclear localization of Nrf2  coincides with increased DNA binding of a putative Nrf2/MafK heterodimer  to its cognate cis-regulatory site, i.e., the antioxidant-responsive element  (ARE).	bind
17800	2	5662	6	10	NULL	NULL	NULL	ARE	GP		is					antioxidant-responsive element	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0540-0549_free-radic-biol-med_39_11_16274879_s_6	16274879	(ii) Nuclear localization of Nrf2  coincides with increased DNA binding of a putative Nrf2/MafK heterodimer  to its cognate cis-regulatory site, i.e., the antioxidant-responsive element  (ARE).	bind
17801	3	5662	6	10	NULL	NULL	NULL	Nrf2	GP	nuclear localization of	increases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0540-0549_free-radic-biol-med_39_11_16274879_s_6	16274879	(ii) Nuclear localization of Nrf2  coincides with increased DNA binding of a putative Nrf2/MafK heterodimer  to its cognate cis-regulatory site, i.e., the antioxidant-responsive element  (ARE).	bind
20315	4	5662	6	10	NULL	NULL	NULL	ARE	GP		is a type of					cis-regulatory site	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0540-0549_free-radic-biol-med_39_11_16274879_s_6	16274879	(ii) Nuclear localization of Nrf2  coincides with increased DNA binding of a putative Nrf2/MafK heterodimer  to its cognate cis-regulatory site, i.e., the antioxidant-responsive element  (ARE).	bind
17161	1	5662	7	10	NULL	NULL	NULL	Nrf2/MafK heterodimer	GP	putative	bind									ARE	NULL		NULL	NULL	NULL	NULL	abs-batch0540-0549_free-radic-biol-med_39_11_16274879_s_6	16274879	(ii) Nuclear localization of Nrf2  coincides with increased DNA binding of a putative Nrf2/MafK heterodimer  to its cognate cis-regulatory site, i.e., the antioxidant-responsive element  (ARE).	bind
17162	2	5662	7	10	NULL	NULL	NULL	Nrf2	GP	Nuclear localization of	increase					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0540-0549_free-radic-biol-med_39_11_16274879_s_6	16274879	(ii) Nuclear localization of Nrf2  coincides with increased DNA binding of a putative Nrf2/MafK heterodimer  to its cognate cis-regulatory site, i.e., the antioxidant-responsive element  (ARE).	bind
17163	3	5662	7	10	NULL	NULL	NULL	ARE	GP		is					antioxidant-responsive element	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0540-0549_free-radic-biol-med_39_11_16274879_s_6	16274879	(ii) Nuclear localization of Nrf2  coincides with increased DNA binding of a putative Nrf2/MafK heterodimer  to its cognate cis-regulatory site, i.e., the antioxidant-responsive element  (ARE).	bind
17164	4	5662	7	10	NULL	NULL	NULL	ARE	GP		is a type of					 cis-regulatory site	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0540-0549_free-radic-biol-med_39_11_16274879_s_6	16274879	(ii) Nuclear localization of Nrf2  coincides with increased DNA binding of a putative Nrf2/MafK heterodimer  to its cognate cis-regulatory site, i.e., the antioxidant-responsive element  (ARE).	bind
17802	1	5663	6	10	NULL	NULL	NULL	p60	GP		bind					ICP0	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-virol_73_5_10196275_s_10	10196275	(ii) p60 also bound ICP0; the binding of ICP0 was independent  of that of ICP22.	bind
17803	2	5663	6	10	NULL	NULL	NULL	ICP0	GP	binding of	is independent of					ICP22	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-virol_73_5_10196275_s_10	10196275	(ii) p60 also bound ICP0; the binding of ICP0 was independent  of that of ICP22.	bind
17165	1	5663	7	10	NULL	NULL	NULL	p60	GP		bind					ICP0	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-virol_73_5_10196275_s_10	10196275	(ii) p60 also bound ICP0; the binding of ICP0 was independent  of that of ICP22.	bind
17166	2	5663	7	10	NULL	NULL	NULL	ICP0	GP	binding of	is independent of					 ICP22	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-virol_73_5_10196275_s_10	10196275	(ii) p60 also bound ICP0; the binding of ICP0 was independent  of that of ICP22.	bind
17804	1	5665	6	10	NULL	NULL	NULL	synapsin I	GP		bind					SV	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_42_43769_s_258	15265868	(ii) Rab3A recruitment by SV in the presence of RabGDI parallels the amount of synapsin I bound to SV.	bind
17805	2	5665	6	10	NULL	NULL	NULL	SV	OrganismPart		recruits					Rab3A	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_42_43769_s_258	15265868	(ii) Rab3A recruitment by SV in the presence of RabGDI parallels the amount of synapsin I bound to SV.	bind
17806	3	5665	6	10	NULL	NULL	NULL	statement 2	Process		occurs in presence of					RabGDI	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_42_43769_s_258	15265868	(ii) Rab3A recruitment by SV in the presence of RabGDI parallels the amount of synapsin I bound to SV.	bind
20316	4	5665	6	10	NULL	NULL	NULL	statement 1	Process		parallels					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_42_43769_s_258	15265868	(ii) Rab3A recruitment by SV in the presence of RabGDI parallels the amount of synapsin I bound to SV.	bind
17170	1	5665	7	10	NULL	NULL	NULL	SV	OrganismPart		recruits					 Rab3A 	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_42_43769_s_258	15265868	(ii) Rab3A recruitment by SV in the presence of RabGDI parallels the amount of synapsin I bound to SV.	bind
17171	2	5665	7	10	NULL	NULL	NULL	statement 1	Process		occurs in the presence of					RabGDI	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_42_43769_s_258	15265868	(ii) Rab3A recruitment by SV in the presence of RabGDI parallels the amount of synapsin I bound to SV.	bind
17172	3	5665	7	10	NULL	NULL	NULL	SV	OrganismPart		bind					synapsin I	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_42_43769_s_258	15265868	(ii) Rab3A recruitment by SV in the presence of RabGDI parallels the amount of synapsin I bound to SV.	bind
17173	4	5665	7	10	NULL	NULL	NULL	statement 1	Process		parallels					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_42_43769_s_258	15265868	(ii) Rab3A recruitment by SV in the presence of RabGDI parallels the amount of synapsin I bound to SV.	bind
17807	1	5666	6	10	NULL	NULL	NULL	fVIII	GP		bind					LRP	GP	purified			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_53_37685_s_250	10608826	(ii) RAP completely inhibits fVIII binding to purified LRP.	bind
17808	2	5666	6	10	NULL	NULL	NULL	RAP	GP		inhibits		completely			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_53_37685_s_250	10608826	(ii) RAP completely inhibits fVIII binding to purified LRP.	bind
17174	1	5666	7	10	NULL	NULL	NULL	fVIII	GP		binds to					LRP	GP	purified			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_53_37685_s_250	10608826	(ii) RAP completely inhibits fVIII binding to purified LRP.	bind
17175	2	5666	7	10	NULL	NULL	NULL	RAP	GP		inhibits		completely			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_53_37685_s_250	10608826	(ii) RAP completely inhibits fVIII binding to purified LRP.	bind
17809	1	5667	6	10	NULL	NULL	NULL	Raf-1	GP		bind					Rb	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_460	15485920	(ii) Rb phosphorylation can be observed when Raf-1, but not cyclin-cdk's, are bound to Rb.	bind
17810	2	5667	6	10	NULL	NULL	NULL	cyclin-cdk	GP		bind					Rb	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_460	15485920	(ii) Rb phosphorylation can be observed when Raf-1, but not cyclin-cdk's, are bound to Rb.	bind
17811	3	5667	6	10	NULL	NULL	NULL	Rb	GP	phosphorylation of	is observed with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_460	15485920	(ii) Rb phosphorylation can be observed when Raf-1, but not cyclin-cdk's, are bound to Rb.	bind
17812	4	5667	6	10	NULL	NULL	NULL	Rb	GP	phosphorylation of	is not observed with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_460	15485920	(ii) Rb phosphorylation can be observed when Raf-1, but not cyclin-cdk's, are bound to Rb.	bind
17176	1	5667	7	10	NULL	NULL	NULL	Raf-1	GP		bind					Rb	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_460	15485920	(ii) Rb phosphorylation can be observed when Raf-1, but not cyclin-cdk's, are bound to Rb.	bind
17177	2	5667	7	10	NULL	NULL	NULL	Rb	GP		undergoes					phosphorylation	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_460	15485920	(ii) Rb phosphorylation can be observed when Raf-1, but not cyclin-cdk's, are bound to Rb.	bind
17178	3	5667	7	10	NULL	NULL	NULL	statement 2	Process		occurs upon					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_460	15485920	(ii) Rb phosphorylation can be observed when Raf-1, but not cyclin-cdk's, are bound to Rb.	bind
17179	4	5667	7	10	NULL	NULL	NULL	cyclin-cdks	GP		bind					Rb	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_460	15485920	(ii) Rb phosphorylation can be observed when Raf-1, but not cyclin-cdk's, are bound to Rb.	bind
20737	5	5667	7	10	NULL	NULL	NULL	Rb	GP		does not					phosphorylation	Process	undergo			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_460	15485920	(ii) Rb phosphorylation can be observed when Raf-1, but not cyclin-cdk's, are bound to Rb.	bind
20738	6	5667	7	10	NULL	NULL	NULL	statement 5	Process		occurs upon					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_21_9527_s_460	15485920	(ii) Rb phosphorylation can be observed when Raf-1, but not cyclin-cdk's, are bound to Rb.	bind
17814	1	5668	6	10	NULL	NULL	NULL	UMSBP	GP	recombinant	bind									H14 sequence	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_19_13419_s_200	10224106	(ii) Recombinant UMSBP, expressed in bacteria by a plasmid carrying the cloned  C. fasciculata  UMSBP gene (and subsequently purified to apparent homogeneity), binds the H14 sequence as efficiently as it binds the UMS (Fig.  3).	bind
17815	2	5668	6	10	NULL	NULL	NULL	UMSBP	GP	recombinant	bind									UMS	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_19_13419_s_200	10224106	(ii) Recombinant UMSBP, expressed in bacteria by a plasmid carrying the cloned  C. fasciculata  UMSBP gene (and subsequently purified to apparent homogeneity), binds the H14 sequence as efficiently as it binds the UMS (Fig.  3).	bind
17816	3	5668	6	10	NULL	NULL	NULL	statement 1	Process		is as efficient as					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_19_13419_s_200	10224106	(ii) Recombinant UMSBP, expressed in bacteria by a plasmid carrying the cloned  C. fasciculata  UMSBP gene (and subsequently purified to apparent homogeneity), binds the H14 sequence as efficiently as it binds the UMS (Fig.  3).	bind
17180	1	5668	7	10	NULL	NULL	NULL	UMSBP	GP	recombinant	binds									H14 sequence 	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_19_13419_s_200	10224106	(ii) Recombinant UMSBP, expressed in bacteria by a plasmid carrying the cloned  C. fasciculata  UMSBP gene (and subsequently purified to apparent homogeneity), binds the H14 sequence as efficiently as it binds the UMS (Fig.  3).	bind
17181	2	5668	7	10	NULL	NULL	NULL	UMSBP	GP	recombinant	bind									UMS	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_19_13419_s_200	10224106	(ii) Recombinant UMSBP, expressed in bacteria by a plasmid carrying the cloned  C. fasciculata  UMSBP gene (and subsequently purified to apparent homogeneity), binds the H14 sequence as efficiently as it binds the UMS (Fig.  3).	bind
17183	4	5668	7	10	NULL	NULL	NULL	statement 1	Process		is as efficient as					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_19_13419_s_200	10224106	(ii) Recombinant UMSBP, expressed in bacteria by a plasmid carrying the cloned  C. fasciculata  UMSBP gene (and subsequently purified to apparent homogeneity), binds the H14 sequence as efficiently as it binds the UMS (Fig.  3).	bind
17818	1	5669	6	10	NULL	NULL	NULL	Sec24D	GP		does not bind					CFP-rGAT1-delta37	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_27_28553_s_488	15073174	(ii) Sec24D did not bind to CFP-rGAT1-delta37.	bind
17184	1	5669	7	10	NULL	NULL	NULL	Sec24D	GP		does not bind					CFP-rGAT1-delta37	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_27_28553_s_488	15073174	(ii) Sec24D did not bind to CFP-rGAT1-delta37.	bind
17819	1	5670	6	10	NULL	NULL	NULL	NELF	GP		bind		sequence specifically			RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2918_s_287	11940650	(ii) Sequence-specific RNA binding by NELF is important for transcription repression, and substitution did not work because RNA-binding specificity is different between NELF-E and CstF-64.	bind
17820	2	5670	6	10	NULL	NULL	NULL	statement 1	Process		is important for					transcription repression	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2918_s_287	11940650	(ii) Sequence-specific RNA binding by NELF is important for transcription repression, and substitution did not work because RNA-binding specificity is different between NELF-E and CstF-64.	bind
20317	3	5670	6	10	NULL	NULL	NULL	NELF-E	GP		bind					RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2918_s_287	11940650	(ii) Sequence-specific RNA binding by NELF is important for transcription repression, and substitution did not work because RNA-binding specificity is different between NELF-E and CstF-64.	bind
20318	4	5670	6	10	NULL	NULL	NULL	CstF-64	GP		bind					RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2918_s_287	11940650	(ii) Sequence-specific RNA binding by NELF is important for transcription repression, and substitution did not work because RNA-binding specificity is different between NELF-E and CstF-64.	bind
20319	5	5670	6	10	NULL	NULL	NULL	statement 3	Process	binding affinity of	is different from					statement 4	Process	binding affinity of 			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2918_s_287	11940650	(ii) Sequence-specific RNA binding by NELF is important for transcription repression, and substitution did not work because RNA-binding specificity is different between NELF-E and CstF-64.	bind
20320	6	5670	6	10	NULL	NULL	NULL	NELF-E	GP		was not substituted for					CstF-64	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2918_s_287	11940650	(ii) Sequence-specific RNA binding by NELF is important for transcription repression, and substitution did not work because RNA-binding specificity is different between NELF-E and CstF-64.	bind
20321	7	5670	6	10	NULL	NULL	NULL	statement 6	Process		because of					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2918_s_287	11940650	(ii) Sequence-specific RNA binding by NELF is important for transcription repression, and substitution did not work because RNA-binding specificity is different between NELF-E and CstF-64.	bind
17185	1	5670	7	10	NULL	NULL	NULL	NELF	GP		bind		sequence specifically			RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2918_s_287	11940650	(ii) Sequence-specific RNA binding by NELF is important for transcription repression, and substitution did not work because RNA-binding specificity is different between NELF-E and CstF-64.	bind
17186	2	5670	7	10	NULL	NULL	NULL	statement 1	Process		is important for					transcription 	Process	repression of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2918_s_287	11940650	(ii) Sequence-specific RNA binding by NELF is important for transcription repression, and substitution did not work because RNA-binding specificity is different between NELF-E and CstF-64.	bind
17192	3	5670	7	10	NULL	NULL	NULL	NELF-E	GP		bind					RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2918_s_287	11940650	(ii) Sequence-specific RNA binding by NELF is important for transcription repression, and substitution did not work because RNA-binding specificity is different between NELF-E and CstF-64.	bind
17193	4	5670	7	10	NULL	NULL	NULL	CstF-64	GP		bind					RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2918_s_287	11940650	(ii) Sequence-specific RNA binding by NELF is important for transcription repression, and substitution did not work because RNA-binding specificity is different between NELF-E and CstF-64.	bind
17194	5	5670	7	10	NULL	NULL	NULL	statement 3	Process		is different from					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2918_s_287	11940650	(ii) Sequence-specific RNA binding by NELF is important for transcription repression, and substitution did not work because RNA-binding specificity is different between NELF-E and CstF-64.	bind
20287	6	5670	7	10	NULL	NULL	NULL	NELF-E	GP		is not substituted for					CstF-64	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2918_s_287	11940650	(ii) Sequence-specific RNA binding by NELF is important for transcription repression, and substitution did not work because RNA-binding specificity is different between NELF-E and CstF-64.	bind
20288	7	5670	7	10	NULL	NULL	NULL	statement 6	Process		because of					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2918_s_287	11940650	(ii) Sequence-specific RNA binding by NELF is important for transcription repression, and substitution did not work because RNA-binding specificity is different between NELF-E and CstF-64.	bind
17889	1	5671	6	10	NULL	NULL	NULL	fibrillin-1	GP		bind					glycosaminoglycan chain	Chemical		sulfated regions		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_36035_s_272	11461921	(ii) Since fibrillin-1 only binds to highly sulfated and iduronated regions within a glycosaminoglycan chain, the patterns of high and low sulfated regions could determine a spatial arrangement of fibrillin-1 necessary to facilitate fibrillin-1 self-interactions or for disulfide bond formation, which is known as one of the initial steps in fibrillin-1 assembly ( 13).	bind
17909	2	5671	6	10	NULL	NULL	NULL	fibrillin-1	GP		interacts with					fibrillin 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_36035_s_272	11461921	(ii) Since fibrillin-1 only binds to highly sulfated and iduronated regions within a glycosaminoglycan chain, the patterns of high and low sulfated regions could determine a spatial arrangement of fibrillin-1 necessary to facilitate fibrillin-1 self-interactions or for disulfide bond formation, which is known as one of the initial steps in fibrillin-1 assembly ( 13).	bind
17910	3	5671	6	10	NULL	NULL	NULL	fibrillin-1	GP	assembly of	requires					disulfide bond	Process	formation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_36035_s_272	11461921	(ii) Since fibrillin-1 only binds to highly sulfated and iduronated regions within a glycosaminoglycan chain, the patterns of high and low sulfated regions could determine a spatial arrangement of fibrillin-1 necessary to facilitate fibrillin-1 self-interactions or for disulfide bond formation, which is known as one of the initial steps in fibrillin-1 assembly ( 13).	bind
18209	4	5671	6	10	NULL	NULL	NULL	fibrillin-1	GP		bind					glycosaminoglycan chain	GP		iduronated regions		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_36035_s_272	11461921	(ii) Since fibrillin-1 only binds to highly sulfated and iduronated regions within a glycosaminoglycan chain, the patterns of high and low sulfated regions could determine a spatial arrangement of fibrillin-1 necessary to facilitate fibrillin-1 self-interactions or for disulfide bond formation, which is known as one of the initial steps in fibrillin-1 assembly ( 13).	bind
17195	1	5671	7	10	NULL	NULL	NULL	fibrillin-1	GP		binds		only			glycosaminoglycan chain	Chemical		highly sulfated within		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_36035_s_272	11461921	(ii) Since fibrillin-1 only binds to highly sulfated and iduronated regions within a glycosaminoglycan chain, the patterns of high and low sulfated regions could determine a spatial arrangement of fibrillin-1 necessary to facilitate fibrillin-1 self-interactions or for disulfide bond formation, which is known as one of the initial steps in fibrillin-1 assembly ( 13).	bind
17196	2	5671	7	10	NULL	NULL	NULL	fibrillin-1	GP		binds		only			glycosaminoglycan chain	Chemical		iduronated regions within		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_36035_s_272	11461921	(ii) Since fibrillin-1 only binds to highly sulfated and iduronated regions within a glycosaminoglycan chain, the patterns of high and low sulfated regions could determine a spatial arrangement of fibrillin-1 necessary to facilitate fibrillin-1 self-interactions or for disulfide bond formation, which is known as one of the initial steps in fibrillin-1 assembly ( 13).	bind
17197	3	5671	7	10	NULL	NULL	NULL			patterns of high and low	determine			sulfated regions		fibrillin-1	GP	spatial arrangement of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_36035_s_272	11461921	(ii) Since fibrillin-1 only binds to highly sulfated and iduronated regions within a glycosaminoglycan chain, the patterns of high and low sulfated regions could determine a spatial arrangement of fibrillin-1 necessary to facilitate fibrillin-1 self-interactions or for disulfide bond formation, which is known as one of the initial steps in fibrillin-1 assembly ( 13).	bind
17198	4	5671	7	10	NULL	NULL	NULL	statement 3	Process		facilitate					fibrillin-1 	GP	self-interactions of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_36035_s_272	11461921	(ii) Since fibrillin-1 only binds to highly sulfated and iduronated regions within a glycosaminoglycan chain, the patterns of high and low sulfated regions could determine a spatial arrangement of fibrillin-1 necessary to facilitate fibrillin-1 self-interactions or for disulfide bond formation, which is known as one of the initial steps in fibrillin-1 assembly ( 13).	bind
17199	5	5671	7	10	NULL	NULL	NULL	statement 3	Process		facilitate					disulfide bond	Process	formation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_36035_s_272	11461921	(ii) Since fibrillin-1 only binds to highly sulfated and iduronated regions within a glycosaminoglycan chain, the patterns of high and low sulfated regions could determine a spatial arrangement of fibrillin-1 necessary to facilitate fibrillin-1 self-interactions or for disulfide bond formation, which is known as one of the initial steps in fibrillin-1 assembly ( 13).	bind
17200	6	5671	7	10	NULL	NULL	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_36035_s_272	11461921	(ii) Since fibrillin-1 only binds to highly sulfated and iduronated regions within a glycosaminoglycan chain, the patterns of high and low sulfated regions could determine a spatial arrangement of fibrillin-1 necessary to facilitate fibrillin-1 self-interactions or for disulfide bond formation, which is known as one of the initial steps in fibrillin-1 assembly ( 13).	bind
17201	7	5671	7	10	NULL	NULL	NULL	statement 4	Process		is					fibrillin-1	GP	initial steps of assembly			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_36035_s_272	11461921	(ii) Since fibrillin-1 only binds to highly sulfated and iduronated regions within a glycosaminoglycan chain, the patterns of high and low sulfated regions could determine a spatial arrangement of fibrillin-1 necessary to facilitate fibrillin-1 self-interactions or for disulfide bond formation, which is known as one of the initial steps in fibrillin-1 assembly ( 13).	bind
17202	8	5671	7	10	NULL	NULL	NULL	statement 5	Process		is					fibrillin-1	GP	initial steps of assembly			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_36035_s_272	11461921	(ii) Since fibrillin-1 only binds to highly sulfated and iduronated regions within a glycosaminoglycan chain, the patterns of high and low sulfated regions could determine a spatial arrangement of fibrillin-1 necessary to facilitate fibrillin-1 self-interactions or for disulfide bond formation, which is known as one of the initial steps in fibrillin-1 assembly ( 13).	bind
17890	1	5672	6	10	NULL	NULL	NULL	Tir	GP		bind					intimin	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_71_4_1725_s_258	12654785	(ii) Subsequent binding of Tir to intimin mediates the intimate attachment between eukaryotic cell and bacterium and (iii) thereby induces a signal which leads to Esp secretion and formation of the type III translocon.	bind
17891	2	5672	6	10	NULL	NULL	NULL	eukaryotic cell	Cell		attaches		intimately			bacterium	Organism				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_71_4_1725_s_258	12654785	(ii) Subsequent binding of Tir to intimin mediates the intimate attachment between eukaryotic cell and bacterium and (iii) thereby induces a signal which leads to Esp secretion and formation of the type III translocon.	bind
17892	3	5672	6	10	NULL	NULL	NULL	statement 1	Process		mediates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_71_4_1725_s_258	12654785	(ii) Subsequent binding of Tir to intimin mediates the intimate attachment between eukaryotic cell and bacterium and (iii) thereby induces a signal which leads to Esp secretion and formation of the type III translocon.	bind
17893	4	5672	6	10	NULL	NULL	NULL	statement 2	Process		signals					Esp	GP	secretion of			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_71_4_1725_s_258	12654785	(ii) Subsequent binding of Tir to intimin mediates the intimate attachment between eukaryotic cell and bacterium and (iii) thereby induces a signal which leads to Esp secretion and formation of the type III translocon.	bind
17894	5	5672	6	10	NULL	NULL	NULL	statement 2	Process		forms					type III translocon	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_71_4_1725_s_258	12654785	(ii) Subsequent binding of Tir to intimin mediates the intimate attachment between eukaryotic cell and bacterium and (iii) thereby induces a signal which leads to Esp secretion and formation of the type III translocon.	bind
17203	1	5672	7	10	NULL	NULL	NULL	Tir	GP		bind					intimin	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_71_4_1725_s_258	12654785	(ii) Subsequent binding of Tir to intimin mediates the intimate attachment between eukaryotic cell and bacterium and (iii) thereby induces a signal which leads to Esp secretion and formation of the type III translocon.	bind
17204	2	5672	7	10	NULL	NULL	NULL	eukaryotic cell	Cell		attaches to		intimately			bacterium	Organism				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_71_4_1725_s_258	12654785	(ii) Subsequent binding of Tir to intimin mediates the intimate attachment between eukaryotic cell and bacterium and (iii) thereby induces a signal which leads to Esp secretion and formation of the type III translocon.	bind
17205	3	5672	7	10	NULL	NULL	NULL	statement 1	Process		mediates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_71_4_1725_s_258	12654785	(ii) Subsequent binding of Tir to intimin mediates the intimate attachment between eukaryotic cell and bacterium and (iii) thereby induces a signal which leads to Esp secretion and formation of the type III translocon.	bind
17206	4	5672	7	10	NULL	NULL	NULL	statement 3	Process		induce a					signal	Process				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_71_4_1725_s_258	12654785	(ii) Subsequent binding of Tir to intimin mediates the intimate attachment between eukaryotic cell and bacterium and (iii) thereby induces a signal which leads to Esp secretion and formation of the type III translocon.	bind
17207	5	5672	7	10	NULL	NULL	NULL	statement 4	Process		leads to					Esp	GP	secretion of			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_71_4_1725_s_258	12654785	(ii) Subsequent binding of Tir to intimin mediates the intimate attachment between eukaryotic cell and bacterium and (iii) thereby induces a signal which leads to Esp secretion and formation of the type III translocon.	bind
17208	6	5672	7	10	NULL	NULL	NULL	statement 4	Process		leads to					type III translocon	GP	formation of			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_71_4_1725_s_258	12654785	(ii) Subsequent binding of Tir to intimin mediates the intimate attachment between eukaryotic cell and bacterium and (iii) thereby induces a signal which leads to Esp secretion and formation of the type III translocon.	bind
17895	1	5673	6	10	NULL	NULL	NULL	putidaredoxin	GP		bind		strongly			CYP101	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_39_36225_s_174	11459837	(ii) The aromatic character of the C-terminal tryptophan in position 106 of putidaredoxin ( 26,  44) is indispensable for the strong binding of putidaredoxin and CYP101, whereas wild type adrenodoxin has no tryptophan at all and also comprises a more extended C-terminal end (adrenodoxin consists of 128 amino acids).	bind
17896	2	5673	6	10	NULL	NULL	NULL	putidaredoxin	GP	aromatic character of	is indspensable for			C-terminal tryptophan		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_39_36225_s_174	11459837	(ii) The aromatic character of the C-terminal tryptophan in position 106 of putidaredoxin ( 26,  44) is indispensable for the strong binding of putidaredoxin and CYP101, whereas wild type adrenodoxin has no tryptophan at all and also comprises a more extended C-terminal end (adrenodoxin consists of 128 amino acids).	bind
22994	3	5673	6	10	NULL	NULL	NULL	adrenodoxin	GP	wild type	does not have					tryptophan	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_39_36225_s_174	11459837	(ii) The aromatic character of the C-terminal tryptophan in position 106 of putidaredoxin ( 26,  44) is indispensable for the strong binding of putidaredoxin and CYP101, whereas wild type adrenodoxin has no tryptophan at all and also comprises a more extended C-terminal end (adrenodoxin consists of 128 amino acids).	bind
22995	4	5673	6	10	NULL	NULL	NULL	adrenodoxin	GP	wild type	comprises of								extended C-terminal end		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_39_36225_s_174	11459837	(ii) The aromatic character of the C-terminal tryptophan in position 106 of putidaredoxin ( 26,  44) is indispensable for the strong binding of putidaredoxin and CYP101, whereas wild type adrenodoxin has no tryptophan at all and also comprises a more extended C-terminal end (adrenodoxin consists of 128 amino acids).	bind
22997	5	5673	6	10	NULL	NULL	NULL	adrenodoxin	GP		consists of								128 amino acids		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_39_36225_s_174	11459837	(ii) The aromatic character of the C-terminal tryptophan in position 106 of putidaredoxin ( 26,  44) is indispensable for the strong binding of putidaredoxin and CYP101, whereas wild type adrenodoxin has no tryptophan at all and also comprises a more extended C-terminal end (adrenodoxin consists of 128 amino acids).	bind
17210	1	5673	7	10	NULL	NULL	NULL	putidaredoxin	GP		binds		strongly			CYP101	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_39_36225_s_174	11459837	(ii) The aromatic character of the C-terminal tryptophan in position 106 of putidaredoxin ( 26,  44) is indispensable for the strong binding of putidaredoxin and CYP101, whereas wild type adrenodoxin has no tryptophan at all and also comprises a more extended C-terminal end (adrenodoxin consists of 128 amino acids).	bind
17211	2	5673	7	10	NULL	NULL	NULL	putidaredoxin	GP	aromatic character of 	is indispensable for			C-terminal tryptophan  position 106		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_39_36225_s_174	11459837	(ii) The aromatic character of the C-terminal tryptophan in position 106 of putidaredoxin ( 26,  44) is indispensable for the strong binding of putidaredoxin and CYP101, whereas wild type adrenodoxin has no tryptophan at all and also comprises a more extended C-terminal end (adrenodoxin consists of 128 amino acids).	bind
17212	3	5673	7	10	NULL	NULL	NULL	adrenodoxin	GP	wild type	does not have					tryptophan	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_39_36225_s_174	11459837	(ii) The aromatic character of the C-terminal tryptophan in position 106 of putidaredoxin ( 26,  44) is indispensable for the strong binding of putidaredoxin and CYP101, whereas wild type adrenodoxin has no tryptophan at all and also comprises a more extended C-terminal end (adrenodoxin consists of 128 amino acids).	bind
17213	4	5673	7	10	NULL	NULL	NULL	adrenodoxin	GP	wild type	comprises of								extended C-terminal end		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_39_36225_s_174	11459837	(ii) The aromatic character of the C-terminal tryptophan in position 106 of putidaredoxin ( 26,  44) is indispensable for the strong binding of putidaredoxin and CYP101, whereas wild type adrenodoxin has no tryptophan at all and also comprises a more extended C-terminal end (adrenodoxin consists of 128 amino acids).	bind
17214	5	5673	7	10	NULL	NULL	NULL	adrenodoxin	GP		consist of								128 amino acids		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_39_36225_s_174	11459837	(ii) The aromatic character of the C-terminal tryptophan in position 106 of putidaredoxin ( 26,  44) is indispensable for the strong binding of putidaredoxin and CYP101, whereas wild type adrenodoxin has no tryptophan at all and also comprises a more extended C-terminal end (adrenodoxin consists of 128 amino acids).	bind
17897	1	5674	6	10	NULL	NULL	NULL	HRI	GP		bind					heme	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_5861_s_357	10454533	(ii) The binding of Hsc70 to transformed HRI may increase the binding affinity of HRI for heme, enhancing the ability of the limiting concentration of heme present in heme-deficient RRL to suppress HRI activation (Fig.  10B,  2).	bind
17898	2	5674	6	10	NULL	NULL	NULL	Hsc70	GP		bind					HRI	GP	transformed			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_5861_s_357	10454533	(ii) The binding of Hsc70 to transformed HRI may increase the binding affinity of HRI for heme, enhancing the ability of the limiting concentration of heme present in heme-deficient RRL to suppress HRI activation (Fig.  10B,  2).	bind
17899	3	5674	6	10	NULL	NULL	NULL	statement 2	Process		increase		may			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_5861_s_357	10454533	(ii) The binding of Hsc70 to transformed HRI may increase the binding affinity of HRI for heme, enhancing the ability of the limiting concentration of heme present in heme-deficient RRL to suppress HRI activation (Fig.  10B,  2).	bind
17900	4	5674	6	10	NULL	NULL	NULL	RRL	GP	heme-deficient	suppress					HRI	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_5861_s_357	10454533	(ii) The binding of Hsc70 to transformed HRI may increase the binding affinity of HRI for heme, enhancing the ability of the limiting concentration of heme present in heme-deficient RRL to suppress HRI activation (Fig.  10B,  2).	bind
17901	5	5674	6	10	NULL	NULL	NULL	statement 3	Process		enhances					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_5861_s_357	10454533	(ii) The binding of Hsc70 to transformed HRI may increase the binding affinity of HRI for heme, enhancing the ability of the limiting concentration of heme present in heme-deficient RRL to suppress HRI activation (Fig.  10B,  2).	bind
17215	1	5674	7	10	NULL	NULL	NULL	Hsc70	GP		bind					HRI	GP	transformed			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_5861_s_357	10454533	(ii) The binding of Hsc70 to transformed HRI may increase the binding affinity of HRI for heme, enhancing the ability of the limiting concentration of heme present in heme-deficient RRL to suppress HRI activation (Fig.  10B,  2).	bind
17216	2	5674	7	10	NULL	NULL	NULL	HRI	GP		bind					heme	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_5861_s_357	10454533	(ii) The binding of Hsc70 to transformed HRI may increase the binding affinity of HRI for heme, enhancing the ability of the limiting concentration of heme present in heme-deficient RRL to suppress HRI activation (Fig.  10B,  2).	bind
17217	3	5674	7	10	NULL	NULL	NULL	statement 1	Process		increase		may			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_5861_s_357	10454533	(ii) The binding of Hsc70 to transformed HRI may increase the binding affinity of HRI for heme, enhancing the ability of the limiting concentration of heme present in heme-deficient RRL to suppress HRI activation (Fig.  10B,  2).	bind
17218	4	5674	7	10	NULL	NULL	NULL	RRL	GP	heme-deficient 	suppress					HRI	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_5861_s_357	10454533	(ii) The binding of Hsc70 to transformed HRI may increase the binding affinity of HRI for heme, enhancing the ability of the limiting concentration of heme present in heme-deficient RRL to suppress HRI activation (Fig.  10B,  2).	bind
17219	5	5674	7	10	NULL	NULL	NULL	statement 3	Process		enhances					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_5861_s_357	10454533	(ii) The binding of Hsc70 to transformed HRI may increase the binding affinity of HRI for heme, enhancing the ability of the limiting concentration of heme present in heme-deficient RRL to suppress HRI activation (Fig.  10B,  2).	bind
17902	1	5675	6	10	NULL	NULL	NULL	mAb 865	GP		bind					HS/heparin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_37_22802_s_145	8798457	(ii) The binding of mAb 865 to HS/heparin decreases with increasing sulfate contents of the polysaccharide.	bind
17903	2	5675	6	10	NULL	NULL	NULL	polysaccharide	Chemical	increasing sulfate contents of	decreases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_37_22802_s_145	8798457	(ii) The binding of mAb 865 to HS/heparin decreases with increasing sulfate contents of the polysaccharide.	bind
17220	1	5675	7	10	NULL	NULL	NULL	mAb 865	GP		bind					HS/heparin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_37_22802_s_145	8798457	(ii) The binding of mAb 865 to HS/heparin decreases with increasing sulfate contents of the polysaccharide.	bind
17221	2	5675	7	10	NULL	NULL	NULL	polysaccharide	Chemical	increasing sulfate contents of	decrease					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_37_22802_s_145	8798457	(ii) The binding of mAb 865 to HS/heparin decreases with increasing sulfate contents of the polysaccharide.	bind
17911	1	5676	6	10	NULL	NULL	NULL	Pd	GP		bind					ferrous CO-P450cam	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2547_s_189	11706033	(ii) The binding of Pd to ferrous CO-P450cam exhibits a 1.5-nm red-shift in the Soret transition.	bind
17222	1	5676	7	10	NULL	NULL	NULL	 Pd	GP		bind					ferrous CO-P450cam	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2547_s_189	11706033	(ii) The binding of Pd to ferrous CO-P450cam exhibits a 1.5-nm red-shift in the Soret transition.	bind
17912	1	5677	6	10	NULL	NULL	NULL	GTP S	GP		does not inhibit					PYY	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_1_574_s_243	8550622	(ii) The inhibition of PYY binding by GTP S could not be observed,  again ruling out a major role of Galpha   in controlling the  dissociation of PYY from PYY receptors.	bind
17913	2	5677	6	10	NULL	NULL	NULL	PYY	GP		dissociates from					PYY receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_1_574_s_243	8550622	(ii) The inhibition of PYY binding by GTP S could not be observed,  again ruling out a major role of Galpha   in controlling the  dissociation of PYY from PYY receptors.	bind
17914	3	5677	6	10	NULL	NULL	NULL	Galpha	GP		does not control					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_1_574_s_243	8550622	(ii) The inhibition of PYY binding by GTP S could not be observed,  again ruling out a major role of Galpha   in controlling the  dissociation of PYY from PYY receptors.	bind
17224	1	5677	7	10	NULL	NULL	NULL	GTP S	GP		does not inhibit					PYY	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_1_574_s_243	8550622	(ii) The inhibition of PYY binding by GTP S could not be observed,  again ruling out a major role of Galpha   in controlling the  dissociation of PYY from PYY receptors.	bind
17225	2	5677	7	10	NULL	NULL	NULL	PYY	GP		dissociates from					PYY receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_1_574_s_243	8550622	(ii) The inhibition of PYY binding by GTP S could not be observed,  again ruling out a major role of Galpha   in controlling the  dissociation of PYY from PYY receptors.	bind
17226	3	5677	7	10	NULL	NULL	NULL	G alpha	GP		does not control					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_1_574_s_243	8550622	(ii) The inhibition of PYY binding by GTP S could not be observed,  again ruling out a major role of Galpha   in controlling the  dissociation of PYY from PYY receptors.	bind
17915	1	5678	6	10	NULL	NULL	NULL	insulin receptor	GP		induces					Stat5B	GP	phosphorylation of	tyrosine		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15985_s_255	10821852	(ii) The insulin receptor induces the tyrosine phosphorylation of Stat5B  in vitro and of Stat3 and Stat5B in cultured cells.	bind
17916	2	5678	6	10	NULL	NULL	NULL	insulin receptor	GP		induces					Stat3	GP	phosphorylation of	tyrosine		NULL	in cultured cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15985_s_255	10821852	(ii) The insulin receptor induces the tyrosine phosphorylation of Stat5B  in vitro and of Stat3 and Stat5B in cultured cells.	bind
17917	3	5678	6	10	NULL	NULL	NULL	insulin receptor	GP		induces					Stat5B	GP	phosphorylation of	tyrosine		NULL	in cultured cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15985_s_255	10821852	(ii) The insulin receptor induces the tyrosine phosphorylation of Stat5B  in vitro and of Stat3 and Stat5B in cultured cells.	bind
17227	1	5678	7	10	NULL	NULL	NULL	insulin receptor	GP		induces					Stat5B	GP	phosphorylation of	tyrosine 		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15985_s_255	10821852	(ii) The insulin receptor induces the tyrosine phosphorylation of Stat5B  in vitro and of Stat3 and Stat5B in cultured cells.	bind
17228	2	5678	7	10	NULL	NULL	NULL	insulin receptor	GP		induces					Stat3	GP	phosphorylation of	tyrosine		NULL	in cultured cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15985_s_255	10821852	(ii) The insulin receptor induces the tyrosine phosphorylation of Stat5B  in vitro and of Stat3 and Stat5B in cultured cells.	bind
17229	3	5678	7	10	NULL	NULL	NULL	insulin receptor	GP		induces					Stat5B	GP	phosphorylation of	tyrosine		NULL	in cultured cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15985_s_255	10821852	(ii) The insulin receptor induces the tyrosine phosphorylation of Stat5B  in vitro and of Stat3 and Stat5B in cultured cells.	bind
17918	1	5680	6	10	NULL	NULL	NULL	Ubr1p	GP		is adjacent to			RING-H2					BRR region		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_23_6832_s_38	10581257	(ii) The RING-H2 domain of Ubr1p, adjacent to the BRR region, is strictly required for ubiquitylation of N-end rule substrates, even though this domain is not required for the binding of Ubr1p to either Ubc2p or N-end rule substrates.	bind
17919	2	5680	6	10	NULL	NULL	NULL	Ubr1p	GP		is required for		strictly	RING-H2		N-end rule substrates	GP	ubiquitination of			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_23_6832_s_38	10581257	(ii) The RING-H2 domain of Ubr1p, adjacent to the BRR region, is strictly required for ubiquitylation of N-end rule substrates, even though this domain is not required for the binding of Ubr1p to either Ubc2p or N-end rule substrates.	bind
17920	3	5680	6	10	NULL	NULL	NULL	Ubr1p	GP		bind					Ubc2p	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_23_6832_s_38	10581257	(ii) The RING-H2 domain of Ubr1p, adjacent to the BRR region, is strictly required for ubiquitylation of N-end rule substrates, even though this domain is not required for the binding of Ubr1p to either Ubc2p or N-end rule substrates.	bind
17921	4	5680	6	10	NULL	NULL	NULL	Ubr1p	GP		is not required for			RING-H2		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_23_6832_s_38	10581257	(ii) The RING-H2 domain of Ubr1p, adjacent to the BRR region, is strictly required for ubiquitylation of N-end rule substrates, even though this domain is not required for the binding of Ubr1p to either Ubc2p or N-end rule substrates.	bind
17922	5	5680	6	10	NULL	NULL	NULL	Ubr1p	GP		bind					N-end rule substrates	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_23_6832_s_38	10581257	(ii) The RING-H2 domain of Ubr1p, adjacent to the BRR region, is strictly required for ubiquitylation of N-end rule substrates, even though this domain is not required for the binding of Ubr1p to either Ubc2p or N-end rule substrates.	bind
17923	6	5680	6	10	NULL	NULL	NULL	Ubr1p	GP		is not required for			RING-H2		statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_23_6832_s_38	10581257	(ii) The RING-H2 domain of Ubr1p, adjacent to the BRR region, is strictly required for ubiquitylation of N-end rule substrates, even though this domain is not required for the binding of Ubr1p to either Ubc2p or N-end rule substrates.	bind
17230	1	5680	7	10	NULL	NULL	NULL	Ubr1p	GP		is required for		strictly	RING-H2 domain		N-end rule substrates	GP	ubiquitylation of			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_23_6832_s_38	10581257	(ii) The RING-H2 domain of Ubr1p, adjacent to the BRR region, is strictly required for ubiquitylation of N-end rule substrates, even though this domain is not required for the binding of Ubr1p to either Ubc2p or N-end rule substrates.	bind
17231	2	5680	7	10	NULL	NULL	NULL	Ubr1p	GP		is adjacent to			RING-H2 domain 					BRR region		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_23_6832_s_38	10581257	(ii) The RING-H2 domain of Ubr1p, adjacent to the BRR region, is strictly required for ubiquitylation of N-end rule substrates, even though this domain is not required for the binding of Ubr1p to either Ubc2p or N-end rule substrates.	bind
17232	3	5680	7	10	NULL	NULL	NULL	Ubr1p	GP		bind					Ubc2p	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_23_6832_s_38	10581257	(ii) The RING-H2 domain of Ubr1p, adjacent to the BRR region, is strictly required for ubiquitylation of N-end rule substrates, even though this domain is not required for the binding of Ubr1p to either Ubc2p or N-end rule substrates.	bind
17233	4	5680	7	10	NULL	NULL	NULL	Ubr1p	GP		bind					N-end rule substrates	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_23_6832_s_38	10581257	(ii) The RING-H2 domain of Ubr1p, adjacent to the BRR region, is strictly required for ubiquitylation of N-end rule substrates, even though this domain is not required for the binding of Ubr1p to either Ubc2p or N-end rule substrates.	bind
17234	5	5680	7	10	NULL	NULL	NULL	Ubr1p	GP		is not required for			RING-H2 domain		statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_23_6832_s_38	10581257	(ii) The RING-H2 domain of Ubr1p, adjacent to the BRR region, is strictly required for ubiquitylation of N-end rule substrates, even though this domain is not required for the binding of Ubr1p to either Ubc2p or N-end rule substrates.	bind
17235	6	5680	7	10	NULL	NULL	NULL	Ubr1p	GP		is not required for			RING-H2 domain 		statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_23_6832_s_38	10581257	(ii) The RING-H2 domain of Ubr1p, adjacent to the BRR region, is strictly required for ubiquitylation of N-end rule substrates, even though this domain is not required for the binding of Ubr1p to either Ubc2p or N-end rule substrates.	bind
17924	2	5681	6	10	NULL	NULL	NULL	statement 1	Process		bind					TMP	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-phys-chem-b-condens-matter-mater-surf-interfaces-biophys_109_1_16851014_s_6	16851014	(ii) The unsaturated UO(2)L(2) complexes with  F ligands bind more strongly TMP than H(2)O, thus preferentially leading  to the UO(2)L(2)(TMP) complex, more hydrophobic than UO(2)L(2)(H(2)O).	bind
18199	3	5681	6	10	NULL	NULL	NULL	statement 1	Process		bind					H(2)O	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-phys-chem-b-condens-matter-mater-surf-interfaces-biophys_109_1_16851014_s_6	16851014	(ii) The unsaturated UO(2)L(2) complexes with  F ligands bind more strongly TMP than H(2)O, thus preferentially leading  to the UO(2)L(2)(TMP) complex, more hydrophobic than UO(2)L(2)(H(2)O).	bind
18200	4	5681	6	10	NULL	NULL	NULL	statement 2	Process		is more stronger than					statement 3	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-phys-chem-b-condens-matter-mater-surf-interfaces-biophys_109_1_16851014_s_6	16851014	(ii) The unsaturated UO(2)L(2) complexes with  F ligands bind more strongly TMP than H(2)O, thus preferentially leading  to the UO(2)L(2)(TMP) complex, more hydrophobic than UO(2)L(2)(H(2)O).	bind
18201	5	5681	6	10	NULL	NULL	NULL	statement 2	Process		forms					UO(2)L(2)(TMP) complex	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-phys-chem-b-condens-matter-mater-surf-interfaces-biophys_109_1_16851014_s_6	16851014	(ii) The unsaturated UO(2)L(2) complexes with  F ligands bind more strongly TMP than H(2)O, thus preferentially leading  to the UO(2)L(2)(TMP) complex, more hydrophobic than UO(2)L(2)(H(2)O).	bind
18202	6	5681	6	10	NULL	NULL	NULL	statement 3	Process		forms					UO(2)L(2)(H(2)O)	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-phys-chem-b-condens-matter-mater-surf-interfaces-biophys_109_1_16851014_s_6	16851014	(ii) The unsaturated UO(2)L(2) complexes with  F ligands bind more strongly TMP than H(2)O, thus preferentially leading  to the UO(2)L(2)(TMP) complex, more hydrophobic than UO(2)L(2)(H(2)O).	bind
18203	7	5681	6	10	NULL	NULL	NULL	statement 5	Process		is more hydrophobic than					statement 6	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-phys-chem-b-condens-matter-mater-surf-interfaces-biophys_109_1_16851014_s_6	16851014	(ii) The unsaturated UO(2)L(2) complexes with  F ligands bind more strongly TMP than H(2)O, thus preferentially leading  to the UO(2)L(2)(TMP) complex, more hydrophobic than UO(2)L(2)(H(2)O).	bind
53245	1	5681	6	10	NULL	NULL	NULL	UO(2)L(2)	Chemical		complexes with					F ligands	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-phys-chem-b-condens-matter-mater-surf-interfaces-biophys_109_1_16851014_s_6	16851014	(ii) The unsaturated UO(2)L(2) complexes with  F ligands bind more strongly TMP than H(2)O, thus preferentially leading  to the UO(2)L(2)(TMP) complex, more hydrophobic than UO(2)L(2)(H(2)O).	bind
17238	1	5681	7	10	NULL	NULL	NULL	UO(2)L(2)	Chemical	unsaturated	complex with					F ligands	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-phys-chem-b-condens-matter-mater-surf-interfaces-biophys_109_1_16851014_s_6	16851014	(ii) The unsaturated UO(2)L(2) complexes with  F ligands bind more strongly TMP than H(2)O, thus preferentially leading  to the UO(2)L(2)(TMP) complex, more hydrophobic than UO(2)L(2)(H(2)O).	bind
17239	2	5681	7	10	NULL	NULL	NULL	statement 1	Process		binds		strongly			TMP	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-phys-chem-b-condens-matter-mater-surf-interfaces-biophys_109_1_16851014_s_6	16851014	(ii) The unsaturated UO(2)L(2) complexes with  F ligands bind more strongly TMP than H(2)O, thus preferentially leading  to the UO(2)L(2)(TMP) complex, more hydrophobic than UO(2)L(2)(H(2)O).	bind
17240	3	5681	7	10	NULL	NULL	NULL	statement 1	Process		binds					H(2)O	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-phys-chem-b-condens-matter-mater-surf-interfaces-biophys_109_1_16851014_s_6	16851014	(ii) The unsaturated UO(2)L(2) complexes with  F ligands bind more strongly TMP than H(2)O, thus preferentially leading  to the UO(2)L(2)(TMP) complex, more hydrophobic than UO(2)L(2)(H(2)O).	bind
17241	4	5681	7	10	NULL	NULL	NULL	statement 2	Process		is stronger than					statement 3	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-phys-chem-b-condens-matter-mater-surf-interfaces-biophys_109_1_16851014_s_6	16851014	(ii) The unsaturated UO(2)L(2) complexes with  F ligands bind more strongly TMP than H(2)O, thus preferentially leading  to the UO(2)L(2)(TMP) complex, more hydrophobic than UO(2)L(2)(H(2)O).	bind
17242	5	5681	7	10	NULL	NULL	NULL	statement 2	Process		leads to					UO(2)L(2)(TMP) complex	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-phys-chem-b-condens-matter-mater-surf-interfaces-biophys_109_1_16851014_s_6	16851014	(ii) The unsaturated UO(2)L(2) complexes with  F ligands bind more strongly TMP than H(2)O, thus preferentially leading  to the UO(2)L(2)(TMP) complex, more hydrophobic than UO(2)L(2)(H(2)O).	bind
17243	6	5681	7	10	NULL	NULL	NULL	statement 3	Process		leads to					UO(2)L(2)(H(2)O)	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-phys-chem-b-condens-matter-mater-surf-interfaces-biophys_109_1_16851014_s_6	16851014	(ii) The unsaturated UO(2)L(2) complexes with  F ligands bind more strongly TMP than H(2)O, thus preferentially leading  to the UO(2)L(2)(TMP) complex, more hydrophobic than UO(2)L(2)(H(2)O).	bind
17244	7	5681	7	10	NULL	NULL	NULL	statement 5	Process		is more hydrophobic than					statement 6	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-phys-chem-b-condens-matter-mater-surf-interfaces-biophys_109_1_16851014_s_6	16851014	(ii) The unsaturated UO(2)L(2) complexes with  F ligands bind more strongly TMP than H(2)O, thus preferentially leading  to the UO(2)L(2)(TMP) complex, more hydrophobic than UO(2)L(2)(H(2)O).	bind
17925	1	5682	6	10	NULL	NULL	NULL	ERK	GP		bind					p38MAPK	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_3_743_s_216	11154262	(ii) Thr403 is situated close to a region that has been proposed to allow the binding of ERK and p38MAPK ( 9,  35).	bind
17245	1	5682	7	10	NULL	NULL	NULL	ERK 	GP		bind					p38MAPK	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_3_743_s_216	11154262	(ii) Thr403 is situated close to a region that has been proposed to allow the binding of ERK and p38MAPK ( 9,  35).	bind
17926	1	5683	6	10	NULL	NULL	NULL	p14ARF	GP		bind					Mdm2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6170_s_243	12167711	(ii) Ubiquitylation of p53, which is blocked upon binding of p14ARF to Mdm2, is permitted by mutant Mdm2.	bind
24574	2	5683	6	10	NULL	NULL	NULL	p14ARF	GP		bind					Mdm2	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6170_s_243	12167711	(ii) Ubiquitylation of p53, which is blocked upon binding of p14ARF to Mdm2, is permitted by mutant Mdm2.	bind
24575	3	5683	6	10	NULL	NULL	NULL	statement 1	Process		blocks					p53	GP	ubiquitylation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6170_s_243	12167711	(ii) Ubiquitylation of p53, which is blocked upon binding of p14ARF to Mdm2, is permitted by mutant Mdm2.	bind
24576	4	5683	6	10	NULL	NULL	NULL	statement 2	Process		allows					p53	GP	ubiquitylation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6170_s_243	12167711	(ii) Ubiquitylation of p53, which is blocked upon binding of p14ARF to Mdm2, is permitted by mutant Mdm2.	bind
17247	1	5683	7	10	NULL	NULL	NULL	p14ARF 	GP		bind					Mdm2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6170_s_243	12167711	(ii) Ubiquitylation of p53, which is blocked upon binding of p14ARF to Mdm2, is permitted by mutant Mdm2.	bind
17248	2	5683	7	10	NULL	NULL	NULL	p14ARF 	GP		bind					Mdm2	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6170_s_243	12167711	(ii) Ubiquitylation of p53, which is blocked upon binding of p14ARF to Mdm2, is permitted by mutant Mdm2.	bind
17249	3	5683	7	10	NULL	NULL	NULL	statement 1	Process		blocks					p53	GP	Ubiquitylation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6170_s_243	12167711	(ii) Ubiquitylation of p53, which is blocked upon binding of p14ARF to Mdm2, is permitted by mutant Mdm2.	bind
17250	4	5683	7	10	NULL	NULL	NULL	statement 2	Process		allows					p53	GP	Ubiquitylation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6170_s_243	12167711	(ii) Ubiquitylation of p53, which is blocked upon binding of p14ARF to Mdm2, is permitted by mutant Mdm2.	bind
17930	1	5685	6	10	NULL	NULL	NULL	kinesin-I	GP		bind					APP	GP	excess			NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_3_389_s_243	11709151	(II) When APP is in excess, kinesin-I binds excess APP, thus titrating kinesin-I from non-APP vesicles, causing non-APP vesicles to stall and inducing a retrograde death signal if an A -containing region is in the organelle jam.	bind
17931	2	5685	6	10	NULL	NULL	NULL	statement 1	Process		cause					non-APP vesicles	CellComponent	stalling of 			NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_3_389_s_243	11709151	(II) When APP is in excess, kinesin-I binds excess APP, thus titrating kinesin-I from non-APP vesicles, causing non-APP vesicles to stall and inducing a retrograde death signal if an A -containing region is in the organelle jam.	bind
17932	3	5685	6	10	NULL	NULL	NULL	statement 1	Process		induces					death signal	Process	retrograde			NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_3_389_s_243	11709151	(II) When APP is in excess, kinesin-I binds excess APP, thus titrating kinesin-I from non-APP vesicles, causing non-APP vesicles to stall and inducing a retrograde death signal if an A -containing region is in the organelle jam.	bind
17934	4	5685	6	10	NULL	NULL	NULL	statement 3	Process		occurs in presence of					A -containing region in organelle jam	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_3_389_s_243	11709151	(II) When APP is in excess, kinesin-I binds excess APP, thus titrating kinesin-I from non-APP vesicles, causing non-APP vesicles to stall and inducing a retrograde death signal if an A -containing region is in the organelle jam.	bind
24577	5	5685	6	10	NULL	NULL	NULL	statement 1	Process		occurs in					APP	GP	excess of			NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_3_389_s_243	11709151	(II) When APP is in excess, kinesin-I binds excess APP, thus titrating kinesin-I from non-APP vesicles, causing non-APP vesicles to stall and inducing a retrograde death signal if an A -containing region is in the organelle jam.	bind
24578	6	5685	6	10	NULL	NULL	NULL	statement 1	Process		titrates					kinesin-I	GP	from non-APP vesicles			NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_3_389_s_243	11709151	(II) When APP is in excess, kinesin-I binds excess APP, thus titrating kinesin-I from non-APP vesicles, causing non-APP vesicles to stall and inducing a retrograde death signal if an A -containing region is in the organelle jam.	bind
17251	1	5685	7	10	NULL	NULL	NULL	kinesin-I	GP		bind					APP	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_3_389_s_243	11709151	(II) When APP is in excess, kinesin-I binds excess APP, thus titrating kinesin-I from non-APP vesicles, causing non-APP vesicles to stall and inducing a retrograde death signal if an A -containing region is in the organelle jam.	bind
17252	2	5685	7	10	NULL	NULL	NULL	statement 1	Process		occur					APP	GP	in excess of			NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_3_389_s_243	11709151	(II) When APP is in excess, kinesin-I binds excess APP, thus titrating kinesin-I from non-APP vesicles, causing non-APP vesicles to stall and inducing a retrograde death signal if an A -containing region is in the organelle jam.	bind
17253	3	5685	7	10	NULL	NULL	NULL	statement 1	Process		titrates					kinesin-I	GP	from non-APP vesicles			NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_3_389_s_243	11709151	(II) When APP is in excess, kinesin-I binds excess APP, thus titrating kinesin-I from non-APP vesicles, causing non-APP vesicles to stall and inducing a retrograde death signal if an A -containing region is in the organelle jam.	bind
17254	4	5685	7	10	NULL	NULL	NULL	statement 1	Process		stall					non-APP vesicles	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_3_389_s_243	11709151	(II) When APP is in excess, kinesin-I binds excess APP, thus titrating kinesin-I from non-APP vesicles, causing non-APP vesicles to stall and inducing a retrograde death signal if an A -containing region is in the organelle jam.	bind
17255	5	5685	7	10	NULL	NULL	NULL	statement 1	Process		induce					death signal	Process	 retrograde			NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_3_389_s_243	11709151	(II) When APP is in excess, kinesin-I binds excess APP, thus titrating kinesin-I from non-APP vesicles, causing non-APP vesicles to stall and inducing a retrograde death signal if an A -containing region is in the organelle jam.	bind
17256	6	5685	7	10	NULL	NULL	NULL	statement 5	Process		occurs in the presence of					A -containing region in organelle jam	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_3_389_s_243	11709151	(II) When APP is in excess, kinesin-I binds excess APP, thus titrating kinesin-I from non-APP vesicles, causing non-APP vesicles to stall and inducing a retrograde death signal if an A -containing region is in the organelle jam.	bind
17936	1	5686	6	10	NULL	NULL	NULL	Nef	GP		bind					Lck	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_11_6333_s_206	8626429	(iii)  What are the consequences of the binding of Nef to Lck?	bind
17361	1	5686	7	10	NULL	NULL	NULL	Nef 	GP		binds					Lck	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_11_6333_s_206	8626429	(iii)  What are the consequences of the binding of Nef to Lck?	bind
17943	1	5687	6	10	NULL	NULL	NULL	ceramide	Chemical		bind					C26 fatty acid	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_23_22515_s_241	15817474	(iii) All mutations that affect fatty acid elongation and the synthesis of the ceramide-bound C26 fatty acid conditionally destabilize newly synthesized Pma1p.	bind
45749	2	5687	6	10	NULL	NULL	NULL	statement 1	Process	mutation of	destabilize		conditionally			Pma1p	GP	newly synthesized			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_23_22515_s_241	15817474	(iii) All mutations that affect fatty acid elongation and the synthesis of the ceramide-bound C26 fatty acid conditionally destabilize newly synthesized Pma1p.	bind
45750	3	5687	6	10	NULL	NULL	NULL	fatty acid elongation	Process	mutation of	destabilize		conditionally			Pma1p	GP	newly synthesized			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_23_22515_s_241	15817474	(iii) All mutations that affect fatty acid elongation and the synthesis of the ceramide-bound C26 fatty acid conditionally destabilize newly synthesized Pma1p.	bind
17257	1	5687	7	10	NULL	NULL	NULL	ceramide	Chemical		bind					C26 fatty acid	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_23_22515_s_241	15817474	(iii) All mutations that affect fatty acid elongation and the synthesis of the ceramide-bound C26 fatty acid conditionally destabilize newly synthesized Pma1p.	bind
17258	2	5687	7	10	NULL	NULL	NULL	mutations	Process		destabilize		conditionally			Pma1p	GP	newly synthesized			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_23_22515_s_241	15817474	(iii) All mutations that affect fatty acid elongation and the synthesis of the ceramide-bound C26 fatty acid conditionally destabilize newly synthesized Pma1p.	bind
17259	3	5687	7	10	NULL	NULL	NULL	mutations	Process		affect					fatty acid	Chemical	elongation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_23_22515_s_241	15817474	(iii) All mutations that affect fatty acid elongation and the synthesis of the ceramide-bound C26 fatty acid conditionally destabilize newly synthesized Pma1p.	bind
17260	4	5687	7	10	NULL	NULL	NULL	mutations	Process		affect					statement 1	Process	synthesis of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_23_22515_s_241	15817474	(iii) All mutations that affect fatty acid elongation and the synthesis of the ceramide-bound C26 fatty acid conditionally destabilize newly synthesized Pma1p.	bind
17261	5	5687	7	10	NULL	NULL	NULL	statement 3	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_23_22515_s_241	15817474	(iii) All mutations that affect fatty acid elongation and the synthesis of the ceramide-bound C26 fatty acid conditionally destabilize newly synthesized Pma1p.	bind
17262	6	5687	7	10	NULL	NULL	NULL	statement 4	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_23_22515_s_241	15817474	(iii) All mutations that affect fatty acid elongation and the synthesis of the ceramide-bound C26 fatty acid conditionally destabilize newly synthesized Pma1p.	bind
17945	1	5688	6	10	NULL	NULL	NULL	ATF-1	GP		bind									CRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_41_25715_s_218	8810350	(iii) ATF-1 bound the major CRE with a lower affinity than CREB.	bind
17946	2	5688	6	10	NULL	NULL	NULL	CREB	GP		bind									CRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_41_25715_s_218	8810350	(iii) ATF-1 bound the major CRE with a lower affinity than CREB.	bind
17948	3	5688	6	10	NULL	NULL	NULL	statement 1	Process		is lower in affinity than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_41_25715_s_218	8810350	(iii) ATF-1 bound the major CRE with a lower affinity than CREB.	bind
17263	1	5688	7	10	NULL	NULL	NULL	ATF-1	GP		bind							major		CRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_41_25715_s_218	8810350	(iii) ATF-1 bound the major CRE with a lower affinity than CREB.	bind
17264	2	5688	7	10	NULL	NULL	NULL	CREB	GP		bind									CRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_41_25715_s_218	8810350	(iii) ATF-1 bound the major CRE with a lower affinity than CREB.	bind
17265	3	5688	7	10	NULL	NULL	NULL	statement 1	Process		has lower affinity than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_41_25715_s_218	8810350	(iii) ATF-1 bound the major CRE with a lower affinity than CREB.	bind
17950	1	5689	6	10	NULL	NULL	NULL	ATP	Chemical		bind					Ssa/sb	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_11_2510_s_226	16688211	(iii) ATP binding to Ssa/sb or Sse1p induces  a transfer of the substrate to Sse1p, before being shuttled to other chaperones such  as TRiC or Hsp90.	bind
17953	2	5689	6	10	NULL	NULL	NULL	ATP	Chemical		bind					Sse1p	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_11_2510_s_226	16688211	(iii) ATP binding to Ssa/sb or Sse1p induces  a transfer of the substrate to Sse1p, before being shuttled to other chaperones such  as TRiC or Hsp90.	bind
17954	3	5689	6	10	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_11_2510_s_226	16688211	(iii) ATP binding to Ssa/sb or Sse1p induces  a transfer of the substrate to Sse1p, before being shuttled to other chaperones such  as TRiC or Hsp90.	bind
17955	4	5689	6	10	NULL	NULL	NULL	statement 1	Process		induces					Sse1p	GP	transfer of substrate to			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_11_2510_s_226	16688211	(iii) ATP binding to Ssa/sb or Sse1p induces  a transfer of the substrate to Sse1p, before being shuttled to other chaperones such  as TRiC or Hsp90.	bind
17956	5	5689	6	10	NULL	NULL	NULL	statement 2	Process		induces					Sse1p	GP	transfer of substrate to			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_11_2510_s_226	16688211	(iii) ATP binding to Ssa/sb or Sse1p induces  a transfer of the substrate to Sse1p, before being shuttled to other chaperones such  as TRiC or Hsp90.	bind
45634	6	5689	6	10	NULL	NULL	NULL	Hsp90	GP		is a type of					chaperone	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_11_2510_s_226	16688211	(iii) ATP binding to Ssa/sb or Sse1p induces  a transfer of the substrate to Sse1p, before being shuttled to other chaperones such  as TRiC or Hsp90.	bind
45635	7	5689	6	10	NULL	NULL	NULL	TRiC	GP		is a type of					chaperone	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_11_2510_s_226	16688211	(iii) ATP binding to Ssa/sb or Sse1p induces  a transfer of the substrate to Sse1p, before being shuttled to other chaperones such  as TRiC or Hsp90.	bind
17266	1	5689	7	10	NULL	NULL	NULL	ATP	Chemical		bind					Ssa/sb 	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_11_2510_s_226	16688211	(iii) ATP binding to Ssa/sb or Sse1p induces  a transfer of the substrate to Sse1p, before being shuttled to other chaperones such  as TRiC or Hsp90.	bind
17267	2	5689	7	10	NULL	NULL	NULL	ATP	Chemical		bind					Sse1p	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_11_2510_s_226	16688211	(iii) ATP binding to Ssa/sb or Sse1p induces  a transfer of the substrate to Sse1p, before being shuttled to other chaperones such  as TRiC or Hsp90.	bind
17268	3	5689	7	10	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_11_2510_s_226	16688211	(iii) ATP binding to Ssa/sb or Sse1p induces  a transfer of the substrate to Sse1p, before being shuttled to other chaperones such  as TRiC or Hsp90.	bind
17269	4	5689	7	10	NULL	NULL	NULL	statement 1	Process		induce					Sse1p	GP	transfer of the substrate to 			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_11_2510_s_226	16688211	(iii) ATP binding to Ssa/sb or Sse1p induces  a transfer of the substrate to Sse1p, before being shuttled to other chaperones such  as TRiC or Hsp90.	bind
17270	5	5689	7	10	NULL	NULL	NULL	statement 2	Process		induce					Sse1p	GP	transfer of the substrate to 			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_11_2510_s_226	16688211	(iii) ATP binding to Ssa/sb or Sse1p induces  a transfer of the substrate to Sse1p, before being shuttled to other chaperones such  as TRiC or Hsp90.	bind
17271	6	5689	7	10	NULL	NULL	NULL	Sse1p	GP		is shuttled to					TRiC	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_11_2510_s_226	16688211	(iii) ATP binding to Ssa/sb or Sse1p induces  a transfer of the substrate to Sse1p, before being shuttled to other chaperones such  as TRiC or Hsp90.	bind
17272	7	5689	7	10	NULL	NULL	NULL	Sse1p	GP		is shuttled to					Hsp90	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_11_2510_s_226	16688211	(iii) ATP binding to Ssa/sb or Sse1p induces  a transfer of the substrate to Sse1p, before being shuttled to other chaperones such  as TRiC or Hsp90.	bind
45633	8	5689	7	10	NULL	NULL	NULL	TRiC	GP		is a type of					chaperone	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_11_2510_s_226	16688211	(iii) ATP binding to Ssa/sb or Sse1p induces  a transfer of the substrate to Sse1p, before being shuttled to other chaperones such  as TRiC or Hsp90.	bind
45636	9	5689	7	10	NULL	NULL	NULL	Hsp90	GP		is a type of					chaperone	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_11_2510_s_226	16688211	(iii) ATP binding to Ssa/sb or Sse1p induces  a transfer of the substrate to Sse1p, before being shuttled to other chaperones such  as TRiC or Hsp90.	bind
17957	1	5690	6	10	NULL	NULL	NULL	ATP	Chemical		bind					cis complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_4_730_s_19	11684006	(iii) ATP bound to the  cis complex acts as a timer, giving the substrate at least 8-10 s to fold inside the cavity after which ATP hydrolysis primes GroES for release from the  cis ring.	bind
17958	2	5690	6	10	NULL	NULL	NULL	GroES	GP		releases from					cis ring	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_4_730_s_19	11684006	(iii) ATP bound to the  cis complex acts as a timer, giving the substrate at least 8-10 s to fold inside the cavity after which ATP hydrolysis primes GroES for release from the  cis ring.	bind
17959	3	5690	6	10	NULL	NULL	NULL	ATP	Chemical	hydrolysis of	primes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_4_730_s_19	11684006	(iii) ATP bound to the  cis complex acts as a timer, giving the substrate at least 8-10 s to fold inside the cavity after which ATP hydrolysis primes GroES for release from the  cis ring.	bind
17961	4	5690	6	10	NULL	NULL	NULL	statement 3	Process		occurs after					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_4_730_s_19	11684006	(iii) ATP bound to the  cis complex acts as a timer, giving the substrate at least 8-10 s to fold inside the cavity after which ATP hydrolysis primes GroES for release from the  cis ring.	bind
17274	1	5690	7	10	NULL	NULL	NULL	ATP	Chemical		bind					cis complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_4_730_s_19	11684006	(iii) ATP bound to the  cis complex acts as a timer, giving the substrate at least 8-10 s to fold inside the cavity after which ATP hydrolysis primes GroES for release from the  cis ring.	bind
17275	2	5690	7	10	NULL	NULL	NULL	GroES	GP		release from					cis ring	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_4_730_s_19	11684006	(iii) ATP bound to the  cis complex acts as a timer, giving the substrate at least 8-10 s to fold inside the cavity after which ATP hydrolysis primes GroES for release from the  cis ring.	bind
23431	3	5690	7	10	NULL	NULL	NULL	ATP	Chemical	hydrolysis of	primes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_4_730_s_19	11684006	(iii) ATP bound to the  cis complex acts as a timer, giving the substrate at least 8-10 s to fold inside the cavity after which ATP hydrolysis primes GroES for release from the  cis ring.	bind
23437	4	5690	7	10	NULL	NULL	NULL	statement 3	Process		occurs after					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_4_730_s_19	11684006	(iii) ATP bound to the  cis complex acts as a timer, giving the substrate at least 8-10 s to fold inside the cavity after which ATP hydrolysis primes GroES for release from the  cis ring.	bind
17962	1	5691	6	10	NULL	NULL	NULL	Msb3	GP		bind					Spa2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8567_s_128	16166638	(iii) Binding of Msb3 and Msb4 to Spa2.	bind
17963	2	5691	6	10	NULL	NULL	NULL	Msb4	GP		bind					Spa2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8567_s_128	16166638	(iii) Binding of Msb3 and Msb4 to Spa2.	bind
17276	1	5691	7	10	NULL	NULL	NULL	Msb3	GP		bind					Spa2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8567_s_128	16166638	(iii) Binding of Msb3 and Msb4 to Spa2.	bind
17277	2	5691	7	10	NULL	NULL	NULL	Msb4	GP		bind					Spa2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8567_s_128	16166638	(iii) Binding of Msb3 and Msb4 to Spa2.	bind
17964	1	5692	6	10	NULL	NULL	NULL				bind			PTB domain		peptides	GP	tyrosine-phosphorylated			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_19_17088_s_156	11877385	(iii) Both PTB domains bind to tyrosine-phosphorylated peptides in an overall enthalpy-driven interaction, which is exemplified by an NP XpY-containing peptide from IL-4R	bind
17278	1	5692	7	10	NULL	NULL	NULL				bind			PTB domain		 peptides	GP	tyrosine-phosphorylated			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_19_17088_s_156	11877385	(iii) Both PTB domains bind to tyrosine-phosphorylated peptides in an overall enthalpy-driven interaction, which is exemplified by an NP XpY-containing peptide from IL-4R	bind
17965	1	5693	6	10	NULL	NULL	NULL	c-Src	GP		phosphorylates					FAK	GP		Tyr-925 site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_45_35624_s_184	10958798	(iii) c-Src then phosphorylates FAK at multiple sites including the Tyr-925 site (for a review see Ref.  46); and (iv) FAK phosphorylation at multiple sites results in conformational changes favoring p130Cas binding to the FAK/c-Src complex ( 29).	bind
17966	2	5693	6	10	NULL	NULL	NULL	p130Cas	GP		bind					FAK/c-Src complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_45_35624_s_184	10958798	(iii) c-Src then phosphorylates FAK at multiple sites including the Tyr-925 site (for a review see Ref.  46); and (iv) FAK phosphorylation at multiple sites results in conformational changes favoring p130Cas binding to the FAK/c-Src complex ( 29).	bind
17967	3	5693	6	10	NULL	NULL	NULL	FAK	GP	phosphorylation of	results in			multiple sites		conformational changes	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_45_35624_s_184	10958798	(iii) c-Src then phosphorylates FAK at multiple sites including the Tyr-925 site (for a review see Ref.  46); and (iv) FAK phosphorylation at multiple sites results in conformational changes favoring p130Cas binding to the FAK/c-Src complex ( 29).	bind
17968	4	5693	6	10	NULL	NULL	NULL	statement 3	Process		favors					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_45_35624_s_184	10958798	(iii) c-Src then phosphorylates FAK at multiple sites including the Tyr-925 site (for a review see Ref.  46); and (iv) FAK phosphorylation at multiple sites results in conformational changes favoring p130Cas binding to the FAK/c-Src complex ( 29).	bind
17280	1	5693	7	10	NULL	NULL	NULL	 c-Src	GP		phosphorylates					FAK 	GP		Tyr-925 site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_45_35624_s_184	10958798	(iii) c-Src then phosphorylates FAK at multiple sites including the Tyr-925 site (for a review see Ref.  46); and (iv) FAK phosphorylation at multiple sites results in conformational changes favoring p130Cas binding to the FAK/c-Src complex ( 29).	bind
17281	2	5693	7	10	NULL	NULL	NULL	c-Src	GP		phosphorylates					FAK 	GP	multiple sites			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_45_35624_s_184	10958798	(iii) c-Src then phosphorylates FAK at multiple sites including the Tyr-925 site (for a review see Ref.  46); and (iv) FAK phosphorylation at multiple sites results in conformational changes favoring p130Cas binding to the FAK/c-Src complex ( 29).	bind
17282	3	5693	7	10	NULL	NULL	NULL	p130Cas	GP		bind					FAK/c-Src complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_45_35624_s_184	10958798	(iii) c-Src then phosphorylates FAK at multiple sites including the Tyr-925 site (for a review see Ref.  46); and (iv) FAK phosphorylation at multiple sites results in conformational changes favoring p130Cas binding to the FAK/c-Src complex ( 29).	bind
17283	4	5693	7	10	NULL	NULL	NULL	statement 2	Process		favors					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_45_35624_s_184	10958798	(iii) c-Src then phosphorylates FAK at multiple sites including the Tyr-925 site (for a review see Ref.  46); and (iv) FAK phosphorylation at multiple sites results in conformational changes favoring p130Cas binding to the FAK/c-Src complex ( 29).	bind
18047	1	5694	6	10	NULL	NULL	NULL	Calmodulin	GP		bind					ER	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_4_1978_s_275	16314411	(iii) Calmodulin binds to the ER in a Ca2+-dependent manner ( ,  ,  ), and this increases the  Kd value of estradiol binding ( ).	bind
18048	2	5694	6	10	NULL	NULL	NULL	statement 1	Process		is dependent on					Ca+2	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_4_1978_s_275	16314411	(iii) Calmodulin binds to the ER in a Ca2+-dependent manner ( ,  ,  ), and this increases the  Kd value of estradiol binding ( ).	bind
17284	1	5694	7	10	NULL	NULL	NULL	Calmodulin	GP		binds					ER	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_4_1978_s_275	16314411	(iii) Calmodulin binds to the ER in a Ca2+-dependent manner ( ,  ,  ), and this increases the  Kd value of estradiol binding ( ).	bind
17285	2	5694	7	10	NULL	NULL	NULL	statement 1	Process		depends on					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_4_1978_s_275	16314411	(iii) Calmodulin binds to the ER in a Ca2+-dependent manner ( ,  ,  ), and this increases the  Kd value of estradiol binding ( ).	bind
18049	1	5695	6	10	NULL	NULL	NULL	D-Xylose	Chemical		bind					XylR	GP				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_64_7_2513_s_196	9647823	(iii) D-Xylose itself binds to XylR, inactivating it to be released from the  xyl operator, thus inducing the  xyl operon.	bind
18050	2	5695	6	10	NULL	NULL	NULL	D-Xylose	Chemical		inactivates					XylR	GP				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_64_7_2513_s_196	9647823	(iii) D-Xylose itself binds to XylR, inactivating it to be released from the  xyl operator, thus inducing the  xyl operon.	bind
18051	3	5695	6	10	NULL	NULL	NULL	XylR	GP		released from					xyl operator	GP				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_64_7_2513_s_196	9647823	(iii) D-Xylose itself binds to XylR, inactivating it to be released from the  xyl operator, thus inducing the  xyl operon.	bind
18052	4	5695	6	10	NULL	NULL	NULL	statement 3	Process		induces					xyl operon	GP				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_64_7_2513_s_196	9647823	(iii) D-Xylose itself binds to XylR, inactivating it to be released from the  xyl operator, thus inducing the  xyl operon.	bind
23014	5	5695	6	10	NULL	NULL	NULL	statement 1	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_64_7_2513_s_196	9647823	(iii) D-Xylose itself binds to XylR, inactivating it to be released from the  xyl operator, thus inducing the  xyl operon.	bind
17286	1	5695	7	10	NULL	NULL	NULL	D-Xylose	Chemical		binds					XylR	GP				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_64_7_2513_s_196	9647823	(iii) D-Xylose itself binds to XylR, inactivating it to be released from the  xyl operator, thus inducing the  xyl operon.	bind
17287	4	5695	7	10	NULL	NULL	NULL	D-Xylose	Chemical		release from					xyl operator	GP			 	NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_64_7_2513_s_196	9647823	(iii) D-Xylose itself binds to XylR, inactivating it to be released from the  xyl operator, thus inducing the  xyl operon.	bind
17288	3	5695	7	10	NULL	NULL	NULL	statement 1	Process		induce					xyl operon	GP			 	NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_64_7_2513_s_196	9647823	(iii) D-Xylose itself binds to XylR, inactivating it to be released from the  xyl operator, thus inducing the  xyl operon.	bind
17289	2	5695	7	10	NULL	NULL	NULL	statement 1	Process		inactivate					XylR	GP				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_64_7_2513_s_196	9647823	(iii) D-Xylose itself binds to XylR, inactivating it to be released from the  xyl operator, thus inducing the  xyl operon.	bind
17290	5	5695	7	10	NULL	NULL	NULL	statement 1	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_64_7_2513_s_196	9647823	(iii) D-Xylose itself binds to XylR, inactivating it to be released from the  xyl operator, thus inducing the  xyl operon.	bind
18053	1	5696	6	10	NULL	NULL	NULL	VLDL	GP		bind					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_biol-chem_386_5_15927888_s_6	15927888	(iii) Different mechanisms specific for a  particular lipoprotein from E3/3 or E2/3 subjects are responsible for  apoE-mediated VLDL binding and apoB-mediated LDL binding to the LDL receptor  in a solid-phase binding assay.	bind
18054	2	5696	6	10	NULL	NULL	NULL	statement 1	Process		is mediated by					apoE	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_biol-chem_386_5_15927888_s_6	15927888	(iii) Different mechanisms specific for a  particular lipoprotein from E3/3 or E2/3 subjects are responsible for  apoE-mediated VLDL binding and apoB-mediated LDL binding to the LDL receptor  in a solid-phase binding assay.	bind
18055	3	5696	6	10	NULL	NULL	NULL	LDL	GP		bind					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_biol-chem_386_5_15927888_s_6	15927888	(iii) Different mechanisms specific for a  particular lipoprotein from E3/3 or E2/3 subjects are responsible for  apoE-mediated VLDL binding and apoB-mediated LDL binding to the LDL receptor  in a solid-phase binding assay.	bind
18056	4	5696	6	10	NULL	NULL	NULL	statement 3	Process		is mediated by					apoB	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_biol-chem_386_5_15927888_s_6	15927888	(iii) Different mechanisms specific for a  particular lipoprotein from E3/3 or E2/3 subjects are responsible for  apoE-mediated VLDL binding and apoB-mediated LDL binding to the LDL receptor  in a solid-phase binding assay.	bind
17291	1	5696	7	10	NULL	NULL	NULL	VLDL	GP		binds					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_biol-chem_386_5_15927888_s_6	15927888	(iii) Different mechanisms specific for a  particular lipoprotein from E3/3 or E2/3 subjects are responsible for  apoE-mediated VLDL binding and apoB-mediated LDL binding to the LDL receptor  in a solid-phase binding assay.	bind
17292	2	5696	7	10	NULL	NULL	NULL	LDL	GP		binds					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_biol-chem_386_5_15927888_s_6	15927888	(iii) Different mechanisms specific for a  particular lipoprotein from E3/3 or E2/3 subjects are responsible for  apoE-mediated VLDL binding and apoB-mediated LDL binding to the LDL receptor  in a solid-phase binding assay.	bind
17293	3	5696	7	10	NULL	NULL	NULL	apoE	Chemical		mediates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_biol-chem_386_5_15927888_s_6	15927888	(iii) Different mechanisms specific for a  particular lipoprotein from E3/3 or E2/3 subjects are responsible for  apoE-mediated VLDL binding and apoB-mediated LDL binding to the LDL receptor  in a solid-phase binding assay.	bind
17294	4	5696	7	10	NULL	NULL	NULL	apoB	Chemical		mediates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_biol-chem_386_5_15927888_s_6	15927888	(iii) Different mechanisms specific for a  particular lipoprotein from E3/3 or E2/3 subjects are responsible for  apoE-mediated VLDL binding and apoB-mediated LDL binding to the LDL receptor  in a solid-phase binding assay.	bind
18057	1	5697	6	10	NULL	NULL	NULL	Ethanol	Chemical		bind		rapidly			p450 2E1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_34_23833_s_175	10446146	(iii) Ethanol binds rapidly to P450 2E1, since burst kinetics are not attenuated when P450 2E1 and ethanol are mixed from separate syringes ( 10).	bind
17295	1	5697	7	10	NULL	NULL	NULL	Ethanol	Chemical		binds		rapidly			P450 2E1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_34_23833_s_175	10446146	(iii) Ethanol binds rapidly to P450 2E1, since burst kinetics are not attenuated when P450 2E1 and ethanol are mixed from separate syringes ( 10).	bind
18058	1	5698	6	10	NULL	NULL	NULL	catenin	GP	expression of	alters					epithelial cell 	Cell	adhesion of			NULL	MDCK cells	NULL	NULL	NULL	NULL	gw70_molcellneurosci_24_3_696_s_147	14664819	(iii) Expression of dominant active forms of  -catenin in MDCK cells altered epithelial  cell adhesion, possibly as a result of  -catenin binding to E-cadherin and APC protein  [ Barth et al., 1997] although other studies suggested that this finding might be specific to certain  cell types [  Loureiro et al., 2001], as overexpression of dominant  -catenin did not alter the cell shape in  Drosophila.	bind
18059	2	5698	6	10	NULL	NULL	NULL	catenin	GP		bind					E-cadherin	GP				NULL	MDCK cells	NULL	NULL	NULL	NULL	gw70_molcellneurosci_24_3_696_s_147	14664819	(iii) Expression of dominant active forms of  -catenin in MDCK cells altered epithelial  cell adhesion, possibly as a result of  -catenin binding to E-cadherin and APC protein  [ Barth et al., 1997] although other studies suggested that this finding might be specific to certain  cell types [  Loureiro et al., 2001], as overexpression of dominant  -catenin did not alter the cell shape in  Drosophila.	bind
18060	3	5698	6	10	NULL	NULL	NULL	catenin	GP		bind					APC protein	GP				NULL	MDCK cells	NULL	NULL	NULL	NULL	gw70_molcellneurosci_24_3_696_s_147	14664819	(iii) Expression of dominant active forms of  -catenin in MDCK cells altered epithelial  cell adhesion, possibly as a result of  -catenin binding to E-cadherin and APC protein  [ Barth et al., 1997] although other studies suggested that this finding might be specific to certain  cell types [  Loureiro et al., 2001], as overexpression of dominant  -catenin did not alter the cell shape in  Drosophila.	bind
18061	4	5698	6	10	NULL	NULL	NULL	catenin	GP	overexpression of	did not alter					cell shape	Process				NULL	drosophila	NULL	NULL	NULL	NULL	gw70_molcellneurosci_24_3_696_s_147	14664819	(iii) Expression of dominant active forms of  -catenin in MDCK cells altered epithelial  cell adhesion, possibly as a result of  -catenin binding to E-cadherin and APC protein  [ Barth et al., 1997] although other studies suggested that this finding might be specific to certain  cell types [  Loureiro et al., 2001], as overexpression of dominant  -catenin did not alter the cell shape in  Drosophila.	bind
23024	5	5698	6	10	NULL	NULL	NULL	statement 2	Process		results in		possibly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_24_3_696_s_147	14664819	(iii) Expression of dominant active forms of  -catenin in MDCK cells altered epithelial  cell adhesion, possibly as a result of  -catenin binding to E-cadherin and APC protein  [ Barth et al., 1997] although other studies suggested that this finding might be specific to certain  cell types [  Loureiro et al., 2001], as overexpression of dominant  -catenin did not alter the cell shape in  Drosophila.	bind
23025	6	5698	6	10	NULL	NULL	NULL	statement 3	Process		results in		possibly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_24_3_696_s_147	14664819	(iii) Expression of dominant active forms of  -catenin in MDCK cells altered epithelial  cell adhesion, possibly as a result of  -catenin binding to E-cadherin and APC protein  [ Barth et al., 1997] although other studies suggested that this finding might be specific to certain  cell types [  Loureiro et al., 2001], as overexpression of dominant  -catenin did not alter the cell shape in  Drosophila.	bind
17296	1	5698	7	10	NULL	NULL	NULL	catenin	GP		bind					 E-cadherin	GP				NULL	MDCK cells 	NULL	NULL	NULL	NULL	gw70_molcellneurosci_24_3_696_s_147	14664819	(iii) Expression of dominant active forms of  -catenin in MDCK cells altered epithelial  cell adhesion, possibly as a result of  -catenin binding to E-cadherin and APC protein  [ Barth et al., 1997] although other studies suggested that this finding might be specific to certain  cell types [  Loureiro et al., 2001], as overexpression of dominant  -catenin did not alter the cell shape in  Drosophila.	bind
17297	2	5698	7	10	NULL	NULL	NULL	catenin	GP		bind					APC protein	GP				NULL	MDCK cells 	NULL	NULL	NULL	NULL	gw70_molcellneurosci_24_3_696_s_147	14664819	(iii) Expression of dominant active forms of  -catenin in MDCK cells altered epithelial  cell adhesion, possibly as a result of  -catenin binding to E-cadherin and APC protein  [ Barth et al., 1997] although other studies suggested that this finding might be specific to certain  cell types [  Loureiro et al., 2001], as overexpression of dominant  -catenin did not alter the cell shape in  Drosophila.	bind
17298	3	5698	7	10	NULL	NULL	NULL	catenin	GP	dominant active forms of	is expressed in					MDCK cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_24_3_696_s_147	14664819	(iii) Expression of dominant active forms of  -catenin in MDCK cells altered epithelial  cell adhesion, possibly as a result of  -catenin binding to E-cadherin and APC protein  [ Barth et al., 1997] although other studies suggested that this finding might be specific to certain  cell types [  Loureiro et al., 2001], as overexpression of dominant  -catenin did not alter the cell shape in  Drosophila.	bind
17299	4	5698	7	10	NULL	NULL	NULL	statement 3	Process		alters					 epithelial cell	Cell	adhesion of			NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_24_3_696_s_147	14664819	(iii) Expression of dominant active forms of  -catenin in MDCK cells altered epithelial  cell adhesion, possibly as a result of  -catenin binding to E-cadherin and APC protein  [ Barth et al., 1997] although other studies suggested that this finding might be specific to certain  cell types [  Loureiro et al., 2001], as overexpression of dominant  -catenin did not alter the cell shape in  Drosophila.	bind
17300	5	5698	7	10	NULL	NULL	NULL	statement 1	Process		results in		possibly			statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_24_3_696_s_147	14664819	(iii) Expression of dominant active forms of  -catenin in MDCK cells altered epithelial  cell adhesion, possibly as a result of  -catenin binding to E-cadherin and APC protein  [ Barth et al., 1997] although other studies suggested that this finding might be specific to certain  cell types [  Loureiro et al., 2001], as overexpression of dominant  -catenin did not alter the cell shape in  Drosophila.	bind
17301	6	5698	7	10	NULL	NULL	NULL	statement 2	Process		results in		possibly			statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_24_3_696_s_147	14664819	(iii) Expression of dominant active forms of  -catenin in MDCK cells altered epithelial  cell adhesion, possibly as a result of  -catenin binding to E-cadherin and APC protein  [ Barth et al., 1997] although other studies suggested that this finding might be specific to certain  cell types [  Loureiro et al., 2001], as overexpression of dominant  -catenin did not alter the cell shape in  Drosophila.	bind
53244	7	5698	7	10	NULL	NULL	NULL	catenin	GP	overexpression of	does not alter					cell shape	Process				NULL	Drosophila	NULL	NULL	NULL	NULL	gw70_molcellneurosci_24_3_696_s_147	14664819	(iii) Expression of dominant active forms of  -catenin in MDCK cells altered epithelial  cell adhesion, possibly as a result of  -catenin binding to E-cadherin and APC protein  [ Barth et al., 1997] although other studies suggested that this finding might be specific to certain  cell types [  Loureiro et al., 2001], as overexpression of dominant  -catenin did not alter the cell shape in  Drosophila.	bind
18062	1	5699	6	10	NULL	NULL	NULL	GM1	Chemical		bind					PDGFR	GP				NULL	in GEM fractions	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_13_11239_s_8	11782461	(iii) GM1 binds with PDGFR in GEM fractions.	bind
17302	1	5699	7	10	NULL	NULL	NULL	GM1	Chemical		bind					PDGFR 	GP				NULL	in GEM fractions	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_13_11239_s_8	11782461	(iii) GM1 binds with PDGFR in GEM fractions.	bind
18063	1	5700	6	10	NULL	NULL	NULL	FLT4L	GP		interact with					PTB-SHC proteins	GP	recombinant			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_12956_s_185	8662748	(iii) GST-PTB SHC recombinant and epitope-tagged SHC proteins were used to confirm this interaction; Tyr1337 mutation (but not Tyr1333 or Tyr1363 mutations) decreased FLT4L capacity to interact with PTB-SHC recombinant proteins, and the deletion of SHC PTB domain (but not of SHC SH2 domain) abolished the binding of SHC to Tyr(P)1337-containing peptide.	bind
18064	2	5700	6	10	NULL	NULL	NULL	FLT4L	GP	mutant	decreases			Tyr1337		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_12956_s_185	8662748	(iii) GST-PTB SHC recombinant and epitope-tagged SHC proteins were used to confirm this interaction; Tyr1337 mutation (but not Tyr1333 or Tyr1363 mutations) decreased FLT4L capacity to interact with PTB-SHC recombinant proteins, and the deletion of SHC PTB domain (but not of SHC SH2 domain) abolished the binding of SHC to Tyr(P)1337-containing peptide.	bind
18065	3	5700	6	10	NULL	NULL	NULL	FLT4L	GP	mutant	does not decrease			Tyr1333		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_12956_s_185	8662748	(iii) GST-PTB SHC recombinant and epitope-tagged SHC proteins were used to confirm this interaction; Tyr1337 mutation (but not Tyr1333 or Tyr1363 mutations) decreased FLT4L capacity to interact with PTB-SHC recombinant proteins, and the deletion of SHC PTB domain (but not of SHC SH2 domain) abolished the binding of SHC to Tyr(P)1337-containing peptide.	bind
18066	4	5700	6	10	NULL	NULL	NULL	FLT4L	GP	mutant	does not decrease			Tyr1363		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_12956_s_185	8662748	(iii) GST-PTB SHC recombinant and epitope-tagged SHC proteins were used to confirm this interaction; Tyr1337 mutation (but not Tyr1333 or Tyr1363 mutations) decreased FLT4L capacity to interact with PTB-SHC recombinant proteins, and the deletion of SHC PTB domain (but not of SHC SH2 domain) abolished the binding of SHC to Tyr(P)1337-containing peptide.	bind
18067	5	5700	6	10	NULL	NULL	NULL	SHC	GP		bind					Tyr(P)1337-containing peptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_12956_s_185	8662748	(iii) GST-PTB SHC recombinant and epitope-tagged SHC proteins were used to confirm this interaction; Tyr1337 mutation (but not Tyr1333 or Tyr1363 mutations) decreased FLT4L capacity to interact with PTB-SHC recombinant proteins, and the deletion of SHC PTB domain (but not of SHC SH2 domain) abolished the binding of SHC to Tyr(P)1337-containing peptide.	bind
18068	6	5700	6	10	NULL	NULL	NULL			deletion of	abolishes			SHC PTB domain		statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_12956_s_185	8662748	(iii) GST-PTB SHC recombinant and epitope-tagged SHC proteins were used to confirm this interaction; Tyr1337 mutation (but not Tyr1333 or Tyr1363 mutations) decreased FLT4L capacity to interact with PTB-SHC recombinant proteins, and the deletion of SHC PTB domain (but not of SHC SH2 domain) abolished the binding of SHC to Tyr(P)1337-containing peptide.	bind
18069	7	5700	6	10	NULL	NULL	NULL			deletion of	does not abolish			SHC SH2 domain		statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_12956_s_185	8662748	(iii) GST-PTB SHC recombinant and epitope-tagged SHC proteins were used to confirm this interaction; Tyr1337 mutation (but not Tyr1333 or Tyr1363 mutations) decreased FLT4L capacity to interact with PTB-SHC recombinant proteins, and the deletion of SHC PTB domain (but not of SHC SH2 domain) abolished the binding of SHC to Tyr(P)1337-containing peptide.	bind
17303	1	5700	7	10	NULL	NULL	NULL	FLT4L	GP		bind					GST-PTB SHC	GP	recombinant			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_12956_s_185	8662748	(iii) GST-PTB SHC recombinant and epitope-tagged SHC proteins were used to confirm this interaction; Tyr1337 mutation (but not Tyr1333 or Tyr1363 mutations) decreased FLT4L capacity to interact with PTB-SHC recombinant proteins, and the deletion of SHC PTB domain (but not of SHC SH2 domain) abolished the binding of SHC to Tyr(P)1337-containing peptide.	bind
17304	2	5700	7	10	NULL	NULL	NULL			mutation of	decrease			Tyr1337		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_12956_s_185	8662748	(iii) GST-PTB SHC recombinant and epitope-tagged SHC proteins were used to confirm this interaction; Tyr1337 mutation (but not Tyr1333 or Tyr1363 mutations) decreased FLT4L capacity to interact with PTB-SHC recombinant proteins, and the deletion of SHC PTB domain (but not of SHC SH2 domain) abolished the binding of SHC to Tyr(P)1337-containing peptide.	bind
17305	3	5700	7	10	NULL	NULL	NULL			mutation	does not affect			Tyr1333		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_12956_s_185	8662748	(iii) GST-PTB SHC recombinant and epitope-tagged SHC proteins were used to confirm this interaction; Tyr1337 mutation (but not Tyr1333 or Tyr1363 mutations) decreased FLT4L capacity to interact with PTB-SHC recombinant proteins, and the deletion of SHC PTB domain (but not of SHC SH2 domain) abolished the binding of SHC to Tyr(P)1337-containing peptide.	bind
17306	4	5700	7	10	NULL	NULL	NULL			mutation	does not affect			Tyr1363		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_12956_s_185	8662748	(iii) GST-PTB SHC recombinant and epitope-tagged SHC proteins were used to confirm this interaction; Tyr1337 mutation (but not Tyr1333 or Tyr1363 mutations) decreased FLT4L capacity to interact with PTB-SHC recombinant proteins, and the deletion of SHC PTB domain (but not of SHC SH2 domain) abolished the binding of SHC to Tyr(P)1337-containing peptide.	bind
17307	5	5700	7	10	NULL	NULL	NULL	SHC 	GP		bind					Tyr(P)1337-containing peptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_12956_s_185	8662748	(iii) GST-PTB SHC recombinant and epitope-tagged SHC proteins were used to confirm this interaction; Tyr1337 mutation (but not Tyr1333 or Tyr1363 mutations) decreased FLT4L capacity to interact with PTB-SHC recombinant proteins, and the deletion of SHC PTB domain (but not of SHC SH2 domain) abolished the binding of SHC to Tyr(P)1337-containing peptide.	bind
17308	6	5700	7	10	NULL	NULL	NULL	SHC	GP	deletion of	abolish			PTB domain		statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_12956_s_185	8662748	(iii) GST-PTB SHC recombinant and epitope-tagged SHC proteins were used to confirm this interaction; Tyr1337 mutation (but not Tyr1333 or Tyr1363 mutations) decreased FLT4L capacity to interact with PTB-SHC recombinant proteins, and the deletion of SHC PTB domain (but not of SHC SH2 domain) abolished the binding of SHC to Tyr(P)1337-containing peptide.	bind
17309	7	5700	7	10	NULL	NULL	NULL	SHC	GP	deletion of	does not affect			SH2 domain		statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_12956_s_185	8662748	(iii) GST-PTB SHC recombinant and epitope-tagged SHC proteins were used to confirm this interaction; Tyr1337 mutation (but not Tyr1333 or Tyr1363 mutations) decreased FLT4L capacity to interact with PTB-SHC recombinant proteins, and the deletion of SHC PTB domain (but not of SHC SH2 domain) abolished the binding of SHC to Tyr(P)1337-containing peptide.	bind
18070	1	5701	6	10	NULL	NULL	NULL	flavin cofactor	Chemical		bind					TcuA	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_15_5479_s_74	16855237	(iii) Identification of the flavin cofactor bound to TcuA.  or flavin analysis, a preparation of TcuA that was not reconstituted with FAD was used.	bind
17310	1	5701	7	10	NULL	NULL	NULL	flavin cofactor	Chemical		bind					TcuA	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_15_5479_s_74	16855237	(iii) Identification of the flavin cofactor bound to TcuA.  or flavin analysis, a preparation of TcuA that was not reconstituted with FAD was used.	bind
18071	1	5702	6	10	NULL	NULL	NULL	UxuR	GP		bind							synthetic		 operator	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_12_3695_s_260	10368143	(iii) In gel retardation assays, MeGlcUAXyl3 was particularly effective in preventing the binding of UxuR to a synthetic operator.	bind
18072	2	5702	6	10	NULL	NULL	NULL	MeGlcUAXyl3	Chemical		prevents					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_12_3695_s_260	10368143	(iii) In gel retardation assays, MeGlcUAXyl3 was particularly effective in preventing the binding of UxuR to a synthetic operator.	bind
17311	1	5702	7	10	NULL	NULL	NULL	UxuR 	GP		bind							synthetic 		operator	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_12_3695_s_260	10368143	(iii) In gel retardation assays, MeGlcUAXyl3 was particularly effective in preventing the binding of UxuR to a synthetic operator.	bind
17312	2	5702	7	10	NULL	NULL	NULL	MeGlcUAXyl3	Chemical		prevents					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_12_3695_s_260	10368143	(iii) In gel retardation assays, MeGlcUAXyl3 was particularly effective in preventing the binding of UxuR to a synthetic operator.	bind
18073	1	5703	6	NULL	NULL	0	NULL	cysteine	NULL		bind	NULL	covalently			Flavin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_12_3336_s_243	10852862	(iii) In the FAD binding pocket of flavocytochrome  c of  A. vinosum, there are a cysteine known to covalently bind flavin and two additional cysteines that form a disulfide bridge ( 9).	bind
18074	2	5703	6	NULL	NULL	0	NULL	statement 1	NULL		occurs in	NULL				flavocytochrome c 	NULL	A. vinosum	FAD binding pocket		NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_12_3336_s_243	10852862	(iii) In the FAD binding pocket of flavocytochrome  c of  A. vinosum, there are a cysteine known to covalently bind flavin and two additional cysteines that form a disulfide bridge ( 9).	bind
18075	3	5703	6	NULL	NULL	0	NULL	cysteine	NULL		forms a 	NULL				disulfide bridge	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_12_3336_s_243	10852862	(iii) In the FAD binding pocket of flavocytochrome  c of  A. vinosum, there are a cysteine known to covalently bind flavin and two additional cysteines that form a disulfide bridge ( 9).	bind
18076	4	5703	6	NULL	NULL	0	NULL	statement 3	NULL		occurs in	NULL				flavocytochrome c	NULL	A. vinosum	FAD binding pocket		NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_12_3336_s_243	10852862	(iii) In the FAD binding pocket of flavocytochrome  c of  A. vinosum, there are a cysteine known to covalently bind flavin and two additional cysteines that form a disulfide bridge ( 9).	bind
17313	1	5703	7	NULL	NULL	NULL	NULL	cysteine	AminoAcid		bind		covalently			flavin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_12_3336_s_243	10852862	(iii) In the FAD binding pocket of flavocytochrome  c of  A. vinosum, there are a cysteine known to covalently bind flavin and two additional cysteines that form a disulfide bridge ( 9).	bind
17314	2	5703	7	NULL	NULL	NULL	NULL	statement 1	Process		present in					flavocytochrome c 	Chemical	A. vinosum	FAD binding pocket		NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_12_3336_s_243	10852862	(iii) In the FAD binding pocket of flavocytochrome  c of  A. vinosum, there are a cysteine known to covalently bind flavin and two additional cysteines that form a disulfide bridge ( 9).	bind
17315	3	5703	7	NULL	NULL	NULL	NULL	cysteines	AminoAcid		form					disulfide bridge	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_12_3336_s_243	10852862	(iii) In the FAD binding pocket of flavocytochrome  c of  A. vinosum, there are a cysteine known to covalently bind flavin and two additional cysteines that form a disulfide bridge ( 9).	bind
23451	4	5703	7	NULL	NULL	NULL	NULL	statement 3	Process		present in					flavocytochrome c 	Chemical	A. vinosum	FAD binding pocket		NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_12_3336_s_243	10852862	(iii) In the FAD binding pocket of flavocytochrome  c of  A. vinosum, there are a cysteine known to covalently bind flavin and two additional cysteines that form a disulfide bridge ( 9).	bind
18077	1	5704	6	NULL	NULL	0	NULL	statin	NULL		bind	NULL				LFA-1	NULL				NULL		0	NULL	NULL	NULL	gw70_atherosclerosis_175_1_83_s_181	15186950	(iii) Inflammatory processes involving bacterial infection and superantigen-induced  T cell activation may profit from treatment with a statin that binds LFA-1 (simvastatin).	bind
18078	2	5704	6	NULL	NULL	0	NULL	LFA-1	NULL		is	NULL				simvastatin	NULL				NULL		0	NULL	NULL	NULL	gw70_atherosclerosis_175_1_83_s_181	15186950	(iii) Inflammatory processes involving bacterial infection and superantigen-induced  T cell activation may profit from treatment with a statin that binds LFA-1 (simvastatin).	bind
18079	3	5704	6	10	NULL	0	NULL	superantigen	NULL		induce	NULL				T cell	NULL	activation of			NULL		NULL	NULL	NULL	NULL	gw70_atherosclerosis_175_1_83_s_181	15186950	(iii) Inflammatory processes involving bacterial infection and superantigen-induced  T cell activation may profit from treatment with a statin that binds LFA-1 (simvastatin).	bind
18080	4	5704	6	NULL	NULL	0	NULL	Inflammatory process	NULL		involve	NULL				bacterial infection	NULL				NULL		0	NULL	NULL	NULL	gw70_atherosclerosis_175_1_83_s_181	15186950	(iii) Inflammatory processes involving bacterial infection and superantigen-induced  T cell activation may profit from treatment with a statin that binds LFA-1 (simvastatin).	bind
18081	5	5704	6	10	NULL	0	NULL	inflammatory processes	NULL		involve	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_atherosclerosis_175_1_83_s_181	15186950	(iii) Inflammatory processes involving bacterial infection and superantigen-induced  T cell activation may profit from treatment with a statin that binds LFA-1 (simvastatin).	bind
18082	6	5704	6	NULL	NULL	0	NULL	statement 4	NULL		profit from	NULL	may			statin	NULL	treatment with			NULL		0	NULL	NULL	NULL	gw70_atherosclerosis_175_1_83_s_181	15186950	(iii) Inflammatory processes involving bacterial infection and superantigen-induced  T cell activation may profit from treatment with a statin that binds LFA-1 (simvastatin).	bind
45751	7	5704	6	10	NULL	0	NULL	statement 5	NULL		profit from	NULL	may			statin	NULL	treatment with			NULL		0	NULL	NULL	NULL	gw70_atherosclerosis_175_1_83_s_181	15186950	(iii) Inflammatory processes involving bacterial infection and superantigen-induced  T cell activation may profit from treatment with a statin that binds LFA-1 (simvastatin).	bind
17319	1	5704	7	NULL	NULL	NULL	NULL	statin	GP		binds					LFA-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_atherosclerosis_175_1_83_s_181	15186950	(iii) Inflammatory processes involving bacterial infection and superantigen-induced  T cell activation may profit from treatment with a statin that binds LFA-1 (simvastatin).	bind
17321	2	5704	7	NULL	NULL	NULL	NULL	LFA-1	GP		is					simvastatin	GP				NULL		NULL	NULL	NULL	NULL	gw70_atherosclerosis_175_1_83_s_181	15186950	(iii) Inflammatory processes involving bacterial infection and superantigen-induced  T cell activation may profit from treatment with a statin that binds LFA-1 (simvastatin).	bind
23452	4	5704	7	NULL	NULL	NULL	NULL	Inflammatory process	Process		involve					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_atherosclerosis_175_1_83_s_181	15186950	(iii) Inflammatory processes involving bacterial infection and superantigen-induced  T cell activation may profit from treatment with a statin that binds LFA-1 (simvastatin).	bind
23453	5	5704	7	NULL	NULL	NULL	NULL	Inflammatory process	Process		involve					bacterial infection	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw70_atherosclerosis_175_1_83_s_181	15186950	(iii) Inflammatory processes involving bacterial infection and superantigen-induced  T cell activation may profit from treatment with a statin that binds LFA-1 (simvastatin).	bind
23454	6	5704	7	NULL	NULL	NULL	NULL	statement 4	Process		profit from		may			statin	GP	treatment with			NULL		NULL	NULL	NULL	NULL	gw70_atherosclerosis_175_1_83_s_181	15186950	(iii) Inflammatory processes involving bacterial infection and superantigen-induced  T cell activation may profit from treatment with a statin that binds LFA-1 (simvastatin).	bind
23455	7	5704	7	NULL	NULL	NULL	NULL	statement 5	Process		profit from		may			statin	GP	treatment with			NULL		NULL	NULL	NULL	NULL	gw70_atherosclerosis_175_1_83_s_181	15186950	(iii) Inflammatory processes involving bacterial infection and superantigen-induced  T cell activation may profit from treatment with a statin that binds LFA-1 (simvastatin).	bind
45851	3	5704	7	NULL	NULL	NULL	NULL	superantigen	GP		induce					T cell	Cell	activation of			NULL		NULL	NULL	NULL	NULL	gw70_atherosclerosis_175_1_83_s_181	15186950	(iii) Inflammatory processes involving bacterial infection and superantigen-induced  T cell activation may profit from treatment with a statin that binds LFA-1 (simvastatin).	bind
18083	1	5705	6	NULL	NULL	0	NULL	Stat3	NULL		exhibits	NULL				DNA binding activity	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15985_s_256	10821852	(iii) Insulin stimulates Stat3 and Stat5 DNA binding activities, and (iv) insulin transactivates a reporter gene containing Stat binding sites.	bind
18084	2	5705	6	NULL	NULL	0	NULL	Stat5	NULL		exhibits	NULL				DNA binding activity	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15985_s_256	10821852	(iii) Insulin stimulates Stat3 and Stat5 DNA binding activities, and (iv) insulin transactivates a reporter gene containing Stat binding sites.	bind
18085	3	5705	6	NULL	NULL	0	NULL	Insulin	NULL		stimulates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15985_s_256	10821852	(iii) Insulin stimulates Stat3 and Stat5 DNA binding activities, and (iv) insulin transactivates a reporter gene containing Stat binding sites.	bind
18086	4	5705	6	NULL	NULL	0	NULL	Insulin	NULL		stimulates	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15985_s_256	10821852	(iii) Insulin stimulates Stat3 and Stat5 DNA binding activities, and (iv) insulin transactivates a reporter gene containing Stat binding sites.	bind
18087	5	5705	6	NULL	NULL	0	NULL	Insulin	NULL		transactivates	NULL				reporter gene	NULL			Stat binding sites	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15985_s_256	10821852	(iii) Insulin stimulates Stat3 and Stat5 DNA binding activities, and (iv) insulin transactivates a reporter gene containing Stat binding sites.	bind
17322	1	5705	7	NULL	NULL	NULL	NULL	Stat3	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15985_s_256	10821852	(iii) Insulin stimulates Stat3 and Stat5 DNA binding activities, and (iv) insulin transactivates a reporter gene containing Stat binding sites.	bind
17324	2	5705	7	NULL	NULL	NULL	NULL	Stat5	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15985_s_256	10821852	(iii) Insulin stimulates Stat3 and Stat5 DNA binding activities, and (iv) insulin transactivates a reporter gene containing Stat binding sites.	bind
17325	3	5705	7	NULL	NULL	NULL	NULL	Insulin	GP		stimulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15985_s_256	10821852	(iii) Insulin stimulates Stat3 and Stat5 DNA binding activities, and (iv) insulin transactivates a reporter gene containing Stat binding sites.	bind
17326	4	5705	7	NULL	NULL	NULL	NULL	Insulin	GP		stimulate					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15985_s_256	10821852	(iii) Insulin stimulates Stat3 and Stat5 DNA binding activities, and (iv) insulin transactivates a reporter gene containing Stat binding sites.	bind
17328	5	5705	7	NULL	NULL	NULL	NULL	Insulin	GP		transactivate					reporter gene	GP			Stat binding sites	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15985_s_256	10821852	(iii) Insulin stimulates Stat3 and Stat5 DNA binding activities, and (iv) insulin transactivates a reporter gene containing Stat binding sites.	bind
18088	1	5706	6	NULL	NULL	0	NULL	Sa-Lrp	NULL		bind	NULL				Sa-Lrp	NULL			control region	NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_13_3661_s_263	10850980	(iii) Like  E. coli Lrp, Sa-Lrp binds to its own control region in a leucine-independent manner, suggestive of leucine-independent autoregulation.	bind
18089	2	5706	6	NULL	NULL	0	NULL	statement 1	NULL		is independent of	NULL				leucine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_13_3661_s_263	10850980	(iii) Like  E. coli Lrp, Sa-Lrp binds to its own control region in a leucine-independent manner, suggestive of leucine-independent autoregulation.	bind
18090	3	5706	6	NULL	NULL	0	NULL	Lrp	NULL	E.coli	bind	NULL				Lrp	NULL	E.coli		control region	NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_13_3661_s_263	10850980	(iii) Like  E. coli Lrp, Sa-Lrp binds to its own control region in a leucine-independent manner, suggestive of leucine-independent autoregulation.	bind
18091	4	5706	6	NULL	NULL	0	NULL	statement 3	NULL		is independent of	NULL				leucine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_13_3661_s_263	10850980	(iii) Like  E. coli Lrp, Sa-Lrp binds to its own control region in a leucine-independent manner, suggestive of leucine-independent autoregulation.	bind
23026	5	5706	6	NULL	NULL	0	NULL	statement 1	NULL		suggests	NULL					NULL	independent autoregulation of	leucine		NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_13_3661_s_263	10850980	(iii) Like  E. coli Lrp, Sa-Lrp binds to its own control region in a leucine-independent manner, suggestive of leucine-independent autoregulation.	bind
23027	6	5706	6	NULL	NULL	0	NULL	statement 3	NULL		suggests	NULL					NULL	independent autoregulation of	leucine		NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_13_3661_s_263	10850980	(iii) Like  E. coli Lrp, Sa-Lrp binds to its own control region in a leucine-independent manner, suggestive of leucine-independent autoregulation.	bind
17331	1	5706	7	NULL	NULL	NULL	NULL	Sa-Lrp	GP		bind					Sa-Lrp	GP			control region	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_13_3661_s_263	10850980	(iii) Like  E. coli Lrp, Sa-Lrp binds to its own control region in a leucine-independent manner, suggestive of leucine-independent autoregulation.	bind
17332	2	5706	7	NULL	NULL	NULL	NULL	statement 1	Process		is independent of					leucine	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_13_3661_s_263	10850980	(iii) Like  E. coli Lrp, Sa-Lrp binds to its own control region in a leucine-independent manner, suggestive of leucine-independent autoregulation.	bind
17333	3	5706	7	NULL	NULL	NULL	NULL	Lrp	GP	E. coli	bind					Lrp	GP	E. coli		control region	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_13_3661_s_263	10850980	(iii) Like  E. coli Lrp, Sa-Lrp binds to its own control region in a leucine-independent manner, suggestive of leucine-independent autoregulation.	bind
17334	4	5706	7	NULL	NULL	NULL	NULL	statement 3	Process		is independent of					leucine	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_13_3661_s_263	10850980	(iii) Like  E. coli Lrp, Sa-Lrp binds to its own control region in a leucine-independent manner, suggestive of leucine-independent autoregulation.	bind
17335	5	5706	7	NULL	NULL	NULL	NULL	statement 2	Process		suggests					leucine	AminoAcid	independent autoregulation of			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_13_3661_s_263	10850980	(iii) Like  E. coli Lrp, Sa-Lrp binds to its own control region in a leucine-independent manner, suggestive of leucine-independent autoregulation.	bind
17336	6	5706	7	NULL	NULL	NULL	NULL	statement 4	Process		suggests					leucine	Aminoacid	independent autoregulation of			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_13_3661_s_263	10850980	(iii) Like  E. coli Lrp, Sa-Lrp binds to its own control region in a leucine-independent manner, suggestive of leucine-independent autoregulation.	bind
18092	1	5707	6	10	NULL	0	NULL	GPVI	NULL	cell-expressed	bind	NULL				convulxin	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_50_52293_s_251	15466473	(iii) Only the combination of 9O12 and 3F8 could strongly impair the binding of cell-expressed GPVI to convulxin.	bind
18093	2	5707	6	NULL	NULL	0	NULL	9O12	NULL		impair	NULL	strongly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_50_52293_s_251	15466473	(iii) Only the combination of 9O12 and 3F8 could strongly impair the binding of cell-expressed GPVI to convulxin.	bind
18124	3	5707	6	NULL	NULL	0	NULL	3F8	NULL		impair	NULL	strongly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_50_52293_s_251	15466473	(iii) Only the combination of 9O12 and 3F8 could strongly impair the binding of cell-expressed GPVI to convulxin.	bind
18125	4	5707	6	NULL	NULL	0	NULL	statement 2	NULL		occurs in combination with	NULL	only			statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_50_52293_s_251	15466473	(iii) Only the combination of 9O12 and 3F8 could strongly impair the binding of cell-expressed GPVI to convulxin.	bind
17337	1	5707	7	NULL	NULL	NULL	NULL	GPVI	GP	cell-expressed	bind					convulxin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_50_52293_s_251	15466473	(iii) Only the combination of 9O12 and 3F8 could strongly impair the binding of cell-expressed GPVI to convulxin.	bind
17338	2	5707	7	NULL	NULL	NULL	NULL	9O12	GP		impair		strongly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_50_52293_s_251	15466473	(iii) Only the combination of 9O12 and 3F8 could strongly impair the binding of cell-expressed GPVI to convulxin.	bind
17339	3	5707	7	NULL	NULL	NULL	NULL	3F8	GP		impair		strongly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_50_52293_s_251	15466473	(iii) Only the combination of 9O12 and 3F8 could strongly impair the binding of cell-expressed GPVI to convulxin.	bind
17340	4	5707	7	NULL	NULL	NULL	NULL	statement 2	Process		occur in combination with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_50_52293_s_251	15466473	(iii) Only the combination of 9O12 and 3F8 could strongly impair the binding of cell-expressed GPVI to convulxin.	bind
18129	1	5708	6	NULL	NULL	0	NULL	BRG1	NULL		bind	NULL	directly			IFITM1	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_10_4476_s_269	15121865	(iii) Our ChIP results demonstrate that BRG1 is directly bound to the IFITM1 promoter both in the absence and in the presence of IFN-alpha (Fig.  6).	bind
17341	1	5708	7	NULL	NULL	NULL	NULL	BRG1	GP		bind		directly			IFITM1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_10_4476_s_269	15121865	(iii) Our ChIP results demonstrate that BRG1 is directly bound to the IFITM1 promoter both in the absence and in the presence of IFN-alpha (Fig.  6).	bind
18134	1	5709	6	NULL	NULL	0	NULL	Pex14p	NULL		bind	NULL				Pex5p	NULL	cargo loaded			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_6_1639_s_586	11865044	(iii) Pex14p can bind to cargo-loaded Pex5p, while Pex13p binds only to unloaded Pex5p, consistent with the notion that Pex14p most likely functions as the initial docking site of Pex5p ( 29).	bind
18135	2	5709	6	NULL	NULL	0	NULL	Pex13p	NULL		bind	NULL	only			Pex5p	NULL	unloaded			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_6_1639_s_586	11865044	(iii) Pex14p can bind to cargo-loaded Pex5p, while Pex13p binds only to unloaded Pex5p, consistent with the notion that Pex14p most likely functions as the initial docking site of Pex5p ( 29).	bind
18138	3	5709	6	NULL	NULL	0	NULL	Pex14	NULL		functions as	NULL	mostly			Pex5p	NULL		docking site		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_6_1639_s_586	11865044	(iii) Pex14p can bind to cargo-loaded Pex5p, while Pex13p binds only to unloaded Pex5p, consistent with the notion that Pex14p most likely functions as the initial docking site of Pex5p ( 29).	bind
17342	1	5709	7	NULL	NULL	NULL	NULL	Pex14p	GP		bind					Pex5p	GP	cargo-loaded			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_6_1639_s_586	11865044	(iii) Pex14p can bind to cargo-loaded Pex5p, while Pex13p binds only to unloaded Pex5p, consistent with the notion that Pex14p most likely functions as the initial docking site of Pex5p ( 29).	bind
17343	2	5709	7	NULL	NULL	NULL	NULL	Pex13p	GP		binds		only			Pex5p	GP	unloaded			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_6_1639_s_586	11865044	(iii) Pex14p can bind to cargo-loaded Pex5p, while Pex13p binds only to unloaded Pex5p, consistent with the notion that Pex14p most likely functions as the initial docking site of Pex5p ( 29).	bind
17344	3	5709	7	NULL	NULL	NULL	NULL	Pex14p	GP		functions as 		mostly			Pex5p	GP		docking site		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_6_1639_s_586	11865044	(iii) Pex14p can bind to cargo-loaded Pex5p, while Pex13p binds only to unloaded Pex5p, consistent with the notion that Pex14p most likely functions as the initial docking site of Pex5p ( 29).	bind
18146	1	5710	6	NULL	NULL	0	NULL	CREB	NULL	phosphorylated	bind	NULL				c- fos	NULL			CRE in 5 regulatory region	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_41_25715_s_187	8810350	(iii) Phosphorylated CREB bound to the major CRE in the c- fos 5  regulatory region results in transcriptional activation.	bind
23036	2	5710	6	NULL	NULL	0	NULL	statement 1	NULL		activates	NULL				transcription	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_41_25715_s_187	8810350	(iii) Phosphorylated CREB bound to the major CRE in the c- fos 5  regulatory region results in transcriptional activation.	bind
17345	1	5710	7	NULL	NULL	NULL	NULL	CREB	GP	phosphorylated 	bind					c- fos	GP	major		CRE in 5 regulatory region of 	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_41_25715_s_187	8810350	(iii) Phosphorylated CREB bound to the major CRE in the c- fos 5  regulatory region results in transcriptional activation.	bind
17346	2	5710	7	NULL	NULL	NULL	NULL	statement 1	Process		activates					transcription 	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_41_25715_s_187	8810350	(iii) Phosphorylated CREB bound to the major CRE in the c- fos 5  regulatory region results in transcriptional activation.	bind
18149	1	5711	6	NULL	NULL	0	NULL	hydrolases	NULL		bind	NULL	noncovalently	C-terminal		ubiquitin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_34_20235_s_19	8702753	(iii) Proteins binding noncovalently to ubiquitin: all C-terminal hydrolases (deubiquitinating enzymes) and an S5 subunit of the 26 S proteasome bind noncovalently to ubiquitin ( 10,  11,  12).	bind
18152	2	5711	6	NULL	NULL	0	NULL	26 S proteasome	NULL		bind	NULL	noncovalently	S5 subunit		ubiquitin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_34_20235_s_19	8702753	(iii) Proteins binding noncovalently to ubiquitin: all C-terminal hydrolases (deubiquitinating enzymes) and an S5 subunit of the 26 S proteasome bind noncovalently to ubiquitin ( 10,  11,  12).	bind
18153	3	5711	6	NULL	NULL	0	NULL	hydrolases	NULL		are	NULL		c-terminal		deubiquitinating enzymes	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_34_20235_s_19	8702753	(iii) Proteins binding noncovalently to ubiquitin: all C-terminal hydrolases (deubiquitinating enzymes) and an S5 subunit of the 26 S proteasome bind noncovalently to ubiquitin ( 10,  11,  12).	bind
17381	1	5711	7	NULL	NULL	NULL	NULL	 hydrolases 	GP		bind		noncovalently	C-terminal		Ubiquitin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_34_20235_s_19	8702753	(iii) Proteins binding noncovalently to ubiquitin: all C-terminal hydrolases (deubiquitinating enzymes) and an S5 subunit of the 26 S proteasome bind noncovalently to ubiquitin ( 10,  11,  12).	bind
17383	2	5711	7	NULL	NULL	NULL	NULL	 26 S proteasome	GP		bind		noncovalently	S5 subunit		Ubiquitin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_34_20235_s_19	8702753	(iii) Proteins binding noncovalently to ubiquitin: all C-terminal hydrolases (deubiquitinating enzymes) and an S5 subunit of the 26 S proteasome bind noncovalently to ubiquitin ( 10,  11,  12).	bind
17385	3	5711	7	NULL	NULL	NULL	NULL	 hydrolases	GP		are			C-terminal		deubiquitinating enzymes	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_34_20235_s_19	8702753	(iii) Proteins binding noncovalently to ubiquitin: all C-terminal hydrolases (deubiquitinating enzymes) and an S5 subunit of the 26 S proteasome bind noncovalently to ubiquitin ( 10,  11,  12).	bind
18154	1	5712	6	10	NULL	0	NULL	ERK2	NULL	purified;;activated	bind	NULL				beta	NULL		carboxy terminal		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_16_13539_s_268	11805112	(iii) Purified activated ERK2 can bind the carboxyl termini of beta and gamma and phosphorylate betaThr-613 and gammaThr-623.	bind
18155	2	5712	6	10	NULL	0	NULL	ERK2	NULL	purified;;activated	bind	NULL				gamma	NULL		carboxy terminal		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_16_13539_s_268	11805112	(iii) Purified activated ERK2 can bind the carboxyl termini of beta and gamma and phosphorylate betaThr-613 and gammaThr-623.	bind
18156	3	5712	6	10	NULL	0	NULL	ERK2	NULL	purified;;activated	phosphorylate	NULL				beta	NULL		Thr-613		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_16_13539_s_268	11805112	(iii) Purified activated ERK2 can bind the carboxyl termini of beta and gamma and phosphorylate betaThr-613 and gammaThr-623.	bind
18158	4	5712	6	10	NULL	0	NULL	ERK2	NULL	purified;;activated	phosphorylate	NULL				gamma	NULL		Thr-623		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_16_13539_s_268	11805112	(iii) Purified activated ERK2 can bind the carboxyl termini of beta and gamma and phosphorylate betaThr-613 and gammaThr-623.	bind
17387	1	5712	7	NULL	NULL	NULL	NULL	ERK2	GP	purified;;activated	bind					beta	GP		carboxyl termini 		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_16_13539_s_268	11805112	(iii) Purified activated ERK2 can bind the carboxyl termini of beta and gamma and phosphorylate betaThr-613 and gammaThr-623.	bind
17388	2	5712	7	NULL	NULL	NULL	NULL	ERK2	GP	purified;;activated	bind					gamma	GP		carboxyl termini 		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_16_13539_s_268	11805112	(iii) Purified activated ERK2 can bind the carboxyl termini of beta and gamma and phosphorylate betaThr-613 and gammaThr-623.	bind
17389	3	5712	7	NULL	NULL	NULL	NULL	ERK2	GP	purified;;activated	phosphorylate					 beta	GP		Thr-613		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_16_13539_s_268	11805112	(iii) Purified activated ERK2 can bind the carboxyl termini of beta and gamma and phosphorylate betaThr-613 and gammaThr-623.	bind
17390	4	5712	7	NULL	NULL	NULL	NULL	ERK2	GP	purified;;activated	phosphorylate					gamma	GP		Thr-623		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_16_13539_s_268	11805112	(iii) Purified activated ERK2 can bind the carboxyl termini of beta and gamma and phosphorylate betaThr-613 and gammaThr-623.	bind
18162	1	5713	6	NULL	NULL	0	NULL	Rab1B	NULL		bind	NULL		CLLL		REP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_23_20379_s_243	11389151	(iii) Rab1B-CLLL binds to REP and is geranylgeranylated on the single cysteine by GGTase II, but it can also be modified in a REP-independent manner by GGTase I. (iv) Rab1B(Y78D)CLLL cannot bind REP but can be geranylgeranylated by GGTase I.	bind
18163	2	5713	6	NULL	NULL	0	NULL	GGTase II	NULL		geranylgeranylate	NULL				Rab1B	NULL		CLLL		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_23_20379_s_243	11389151	(iii) Rab1B-CLLL binds to REP and is geranylgeranylated on the single cysteine by GGTase II, but it can also be modified in a REP-independent manner by GGTase I. (iv) Rab1B(Y78D)CLLL cannot bind REP but can be geranylgeranylated by GGTase I.	bind
18164	3	5713	6	NULL	NULL	0	NULL	Rab1B	NULL	mutant	does not bind	NULL		CLLL;;Y78D		REP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_23_20379_s_243	11389151	(iii) Rab1B-CLLL binds to REP and is geranylgeranylated on the single cysteine by GGTase II, but it can also be modified in a REP-independent manner by GGTase I. (iv) Rab1B(Y78D)CLLL cannot bind REP but can be geranylgeranylated by GGTase I.	bind
18165	4	5713	6	NULL	NULL	0	NULL	GGTase I	NULL		geranylgeranylate	NULL				Rab1B	NULL	mutant	Y78D;;CLLL		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_23_20379_s_243	11389151	(iii) Rab1B-CLLL binds to REP and is geranylgeranylated on the single cysteine by GGTase II, but it can also be modified in a REP-independent manner by GGTase I. (iv) Rab1B(Y78D)CLLL cannot bind REP but can be geranylgeranylated by GGTase I.	bind
23037	5	5713	6	NULL	NULL	0	NULL	statement 2	NULL		is independent of	NULL				REP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_23_20379_s_243	11389151	(iii) Rab1B-CLLL binds to REP and is geranylgeranylated on the single cysteine by GGTase II, but it can also be modified in a REP-independent manner by GGTase I. (iv) Rab1B(Y78D)CLLL cannot bind REP but can be geranylgeranylated by GGTase I.	bind
23038	6	5713	6	NULL	NULL	0	NULL	GGTase II	NULL		geranylgeranylates	NULL				statement 1	NULL		single cysteine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_23_20379_s_243	11389151	(iii) Rab1B-CLLL binds to REP and is geranylgeranylated on the single cysteine by GGTase II, but it can also be modified in a REP-independent manner by GGTase I. (iv) Rab1B(Y78D)CLLL cannot bind REP but can be geranylgeranylated by GGTase I.	bind
17394	1	5713	7	NULL	NULL	NULL	NULL	Rab1B	GP		binds			CLLL		REP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_23_20379_s_243	11389151	(iii) Rab1B-CLLL binds to REP and is geranylgeranylated on the single cysteine by GGTase II, but it can also be modified in a REP-independent manner by GGTase I. (iv) Rab1B(Y78D)CLLL cannot bind REP but can be geranylgeranylated by GGTase I.	bind
17395	2	5713	7	NULL	NULL	NULL	NULL	GGTase II	GP		geranylgeranylates					statement 1	Process		single cysteine 		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_23_20379_s_243	11389151	(iii) Rab1B-CLLL binds to REP and is geranylgeranylated on the single cysteine by GGTase II, but it can also be modified in a REP-independent manner by GGTase I. (iv) Rab1B(Y78D)CLLL cannot bind REP but can be geranylgeranylated by GGTase I.	bind
17397	3	5713	7	NULL	NULL	NULL	NULL	GGTase I	GP		geranylgeranylates					Rab1B	GP		CLLL		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_23_20379_s_243	11389151	(iii) Rab1B-CLLL binds to REP and is geranylgeranylated on the single cysteine by GGTase II, but it can also be modified in a REP-independent manner by GGTase I. (iv) Rab1B(Y78D)CLLL cannot bind REP but can be geranylgeranylated by GGTase I.	bind
17398	4	5713	7	NULL	NULL	NULL	NULL	statement 3	Process		is independent of					REP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_23_20379_s_243	11389151	(iii) Rab1B-CLLL binds to REP and is geranylgeranylated on the single cysteine by GGTase II, but it can also be modified in a REP-independent manner by GGTase I. (iv) Rab1B(Y78D)CLLL cannot bind REP but can be geranylgeranylated by GGTase I.	bind
17399	5	5713	7	NULL	NULL	NULL	NULL	Rab1B	GP	mutant	does not bind			CLLL;;Y78D		REP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_23_20379_s_243	11389151	(iii) Rab1B-CLLL binds to REP and is geranylgeranylated on the single cysteine by GGTase II, but it can also be modified in a REP-independent manner by GGTase I. (iv) Rab1B(Y78D)CLLL cannot bind REP but can be geranylgeranylated by GGTase I.	bind
17402	6	5713	7	NULL	NULL	NULL	NULL	GGTase I	GP		geranylgeranylates					Rab1B	GP	mutant	CLLL;;Y78D		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_23_20379_s_243	11389151	(iii) Rab1B-CLLL binds to REP and is geranylgeranylated on the single cysteine by GGTase II, but it can also be modified in a REP-independent manner by GGTase I. (iv) Rab1B(Y78D)CLLL cannot bind REP but can be geranylgeranylated by GGTase I.	bind
18166	1	5714	6	10	NULL	0	NULL	CnNK-2	NULL	recombinant	bind	NULL	sequence specifically			CnNk-2	NULL			NK-2 sites	NULL		NULL	NULL	NULL	NULL	gw70_mechdev_121_2_195_s_165	15037320	(iii) Recombinant  CnNK-2 is binding to NK-2 sites of the  CnNk-2 as well as the  pedibin 5  flanking region in a sequence specific manner ( Fig. 2C,E).	bind
18167	2	5714	6	10	NULL	0	NULL	CnNK-2	NULL	recombinant	bind	NULL	sequence specifically			pedibin	NULL			5 flanking region	NULL		NULL	NULL	NULL	NULL	gw70_mechdev_121_2_195_s_165	15037320	(iii) Recombinant  CnNK-2 is binding to NK-2 sites of the  CnNk-2 as well as the  pedibin 5  flanking region in a sequence specific manner ( Fig. 2C,E).	bind
17403	1	5714	7	NULL	NULL	NULL	NULL	CnNK-2	GP	recombinant	bind		sequence specifically			CnNk-2 	GP			NK-2 sites 	NULL		NULL	NULL	NULL	NULL	gw70_mechdev_121_2_195_s_165	15037320	(iii) Recombinant  CnNK-2 is binding to NK-2 sites of the  CnNk-2 as well as the  pedibin 5  flanking region in a sequence specific manner ( Fig. 2C,E).	bind
17404	2	5714	7	NULL	NULL	NULL	NULL	CnNK-2	GP	recombinant	bind		sequence specifically			pedibin	GP			5 flanking region	NULL		NULL	NULL	NULL	NULL	gw70_mechdev_121_2_195_s_165	15037320	(iii) Recombinant  CnNK-2 is binding to NK-2 sites of the  CnNk-2 as well as the  pedibin 5  flanking region in a sequence specific manner ( Fig. 2C,E).	bind
18169	1	5715	6	NULL	NULL	0	NULL	Rheb	NULL		does not bind	NULL		S20N		guanine nucleotide	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_18_7965_s_284	15340059	(iii) Rheb-S20N does not function as a dominant-negative mutant although Rheb-S20N does not bind the guanine nucleotide.	bind
23039	2	5715	6	NULL	NULL	0	NULL	Rheb	NULL		does not function as	NULL		S20N		dominant-negative mutant	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_18_7965_s_284	15340059	(iii) Rheb-S20N does not function as a dominant-negative mutant although Rheb-S20N does not bind the guanine nucleotide.	bind
17406	1	5715	7	NULL	NULL	NULL	NULL	Rheb	GP		does not bind			S20N		guanine nucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_18_7965_s_284	15340059	(iii) Rheb-S20N does not function as a dominant-negative mutant although Rheb-S20N does not bind the guanine nucleotide.	bind
17407	2	5715	7	NULL	NULL	NULL	NULL	Rheb	GP		does not function as			S20N		dominant negative mutant	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_18_7965_s_284	15340059	(iii) Rheb-S20N does not function as a dominant-negative mutant although Rheb-S20N does not bind the guanine nucleotide.	bind
23040	1	5716	6	NULL	NULL	0	NULL	RhlB 	NULL		bind	NULL				RNase E	NULL				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_15_4189_s_50	16935881	(iii) RhlB is  inactive as a helicase unless it binds RNase E or a fragment thereof (in blue) carrying  an arginine-rich region.	bind
23041	2	5716	6	NULL	NULL	0	NULL	RhlB	NULL		bind	NULL				fragment 	NULL		arginine-rich region		NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_15_4189_s_50	16935881	(iii) RhlB is  inactive as a helicase unless it binds RNase E or a fragment thereof (in blue) carrying  an arginine-rich region.	bind
23043	3	5716	6	NULL	NULL	0	NULL	statement 1	NULL		abolishes	NULL				RhlB helicase	NULL	inactivity of 			NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_15_4189_s_50	16935881	(iii) RhlB is  inactive as a helicase unless it binds RNase E or a fragment thereof (in blue) carrying  an arginine-rich region.	bind
23044	4	5716	6	NULL	NULL	0	NULL	statement 2	NULL		abolishes	NULL				RhlB helicase	NULL	inactivity of			NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_15_4189_s_50	16935881	(iii) RhlB is  inactive as a helicase unless it binds RNase E or a fragment thereof (in blue) carrying  an arginine-rich region.	bind
45755	5	5716	6	10	NULL	0	NULL	statement 3	NULL		is an alternative to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_34_15_4189_s_50	16935881	(iii) RhlB is  inactive as a helicase unless it binds RNase E or a fragment thereof (in blue) carrying  an arginine-rich region.	bind
17408	1	5716	7	NULL	NULL	NULL	NULL	RhlB	GP		bind					RNase E	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_15_4189_s_50	16935881	(iii) RhlB is  inactive as a helicase unless it binds RNase E or a fragment thereof (in blue) carrying  an arginine-rich region.	bind
17409	2	5716	7	NULL	NULL	NULL	NULL	RhlB	GP		bind					fragment	AminoAcid		arginine-rich region		NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_15_4189_s_50	16935881	(iii) RhlB is  inactive as a helicase unless it binds RNase E or a fragment thereof (in blue) carrying  an arginine-rich region.	bind
17410	3	5716	7	NULL	NULL	NULL	NULL	statement 1	Process		abolishes					Rh1B helicase	GP	inactivity of			NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_15_4189_s_50	16935881	(iii) RhlB is  inactive as a helicase unless it binds RNase E or a fragment thereof (in blue) carrying  an arginine-rich region.	bind
45852	4	5716	7	NULL	NULL	NULL	NULL	statement 2	Process		abolishes					RhlB helicase	GP	inactivity of			NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_15_4189_s_50	16935881	(iii) RhlB is  inactive as a helicase unless it binds RNase E or a fragment thereof (in blue) carrying  an arginine-rich region.	bind
18170	1	5717	6	NULL	NULL	0	NULL	Rit	NULL		bind	NULL				B- Raf isoform	NULL	neuronal			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_2_830_s_420	15632082	(iii) Rit demonstrates isoform-specific Raf kinase binding and activation, associating with and activating the neuronal B-Raf isoform, but not C-Raf, explaining its cell type-specific activation of the ERK MAP kinase cascade.	bind
18171	2	5717	6	NULL	NULL	0	NULL	Rit	NULL		activates	NULL				B- Raf isoform	NULL	neuronal			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_2_830_s_420	15632082	(iii) Rit demonstrates isoform-specific Raf kinase binding and activation, associating with and activating the neuronal B-Raf isoform, but not C-Raf, explaining its cell type-specific activation of the ERK MAP kinase cascade.	bind
18172	3	5717	6	NULL	NULL	0	NULL	Rit	NULL		does not bind	NULL				C-Raf	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_2_830_s_420	15632082	(iii) Rit demonstrates isoform-specific Raf kinase binding and activation, associating with and activating the neuronal B-Raf isoform, but not C-Raf, explaining its cell type-specific activation of the ERK MAP kinase cascade.	bind
18173	4	5717	6	NULL	NULL	0	NULL	Rit	NULL		does not activate	NULL				C-Raf	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_2_830_s_420	15632082	(iii) Rit demonstrates isoform-specific Raf kinase binding and activation, associating with and activating the neuronal B-Raf isoform, but not C-Raf, explaining its cell type-specific activation of the ERK MAP kinase cascade.	bind
23046	5	5717	6	NULL	NULL	0	NULL	Rit	NULL		activates	NULL				ERK MAP kinase cascade	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_2_830_s_420	15632082	(iii) Rit demonstrates isoform-specific Raf kinase binding and activation, associating with and activating the neuronal B-Raf isoform, but not C-Raf, explaining its cell type-specific activation of the ERK MAP kinase cascade.	bind
17413	1	5717	7	NULL	NULL	NULL	NULL	Rit	GP		bind					B-Raf isoform	GP	neuronal			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_2_830_s_420	15632082	(iii) Rit demonstrates isoform-specific Raf kinase binding and activation, associating with and activating the neuronal B-Raf isoform, but not C-Raf, explaining its cell type-specific activation of the ERK MAP kinase cascade.	bind
17414	2	5717	7	NULL	NULL	NULL	NULL	Rit	GP		activate					B-Raf isoform	GP	neuronal			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_2_830_s_420	15632082	(iii) Rit demonstrates isoform-specific Raf kinase binding and activation, associating with and activating the neuronal B-Raf isoform, but not C-Raf, explaining its cell type-specific activation of the ERK MAP kinase cascade.	bind
17416	3	5717	7	NULL	NULL	NULL	NULL	Rit	GP		does not bind					C-Raf	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_2_830_s_420	15632082	(iii) Rit demonstrates isoform-specific Raf kinase binding and activation, associating with and activating the neuronal B-Raf isoform, but not C-Raf, explaining its cell type-specific activation of the ERK MAP kinase cascade.	bind
17417	5	5717	7	NULL	NULL	NULL	NULL	Rit	GP 		activates					ERK MAP Kinase cascade	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_2_830_s_420	15632082	(iii) Rit demonstrates isoform-specific Raf kinase binding and activation, associating with and activating the neuronal B-Raf isoform, but not C-Raf, explaining its cell type-specific activation of the ERK MAP kinase cascade.	bind
24953	4	5717	7	NULL	NULL	NULL	NULL	Rit	GP		does not activate					C-Raf	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_2_830_s_420	15632082	(iii) Rit demonstrates isoform-specific Raf kinase binding and activation, associating with and activating the neuronal B-Raf isoform, but not C-Raf, explaining its cell type-specific activation of the ERK MAP kinase cascade.	bind
18174	1	5718	6	NULL	NULL	0	NULL	ScoC	NULL		bind	NULL				aprE	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_10_3056_s_254	15126467	(iii) ScoC binds to the  aprE promoter, but its inhibitory function might be counteracted by a positive factor(s).	bind
18175	2	5718	6	NULL	NULL	0	NULL	ScoC	NULL		inhibits	NULL				aprE	NULL			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_10_3056_s_254	15126467	(iii) ScoC binds to the  aprE promoter, but its inhibitory function might be counteracted by a positive factor(s).	bind
18176	3	5718	6	NULL	NULL	0	NULL	statement 2	NULL		be counteracted by	NULL	might			positive factor	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_10_3056_s_254	15126467	(iii) ScoC binds to the  aprE promoter, but its inhibitory function might be counteracted by a positive factor(s).	bind
17418	1	5718	7	NULL	NULL	NULL	NULL	ScoC	GP		binds to					aprE	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_10_3056_s_254	15126467	(iii) ScoC binds to the  aprE promoter, but its inhibitory function might be counteracted by a positive factor(s).	bind
24954	2	5718	7	NULL	NULL	NULL	NULL	 ScoC	GP		inhibits					aprE	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_10_3056_s_254	15126467	(iii) ScoC binds to the  aprE promoter, but its inhibitory function might be counteracted by a positive factor(s).	bind
24955	3	5718	7	NULL	NULL	NULL	NULL	statement 2	Process		be counter acted by		might			positive factor(s)	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_10_3056_s_254	15126467	(iii) ScoC binds to the  aprE promoter, but its inhibitory function might be counteracted by a positive factor(s).	bind
18177	1	5719	6	NULL	NULL	0	NULL	transcription factors	NULL		bind	NULL	sequence specifically			DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_17_10236_s_163	7730328	(iii) Sequence-specific DNA binding of  transcription factors is clearly estatablished  ( 57) .	bind
17419	1	5719	7	NULL	NULL	NULL	NULL	 transcription factors 	GP		bind		sequence-specifically			DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_17_10236_s_163	7730328	(iii) Sequence-specific DNA binding of  transcription factors is clearly estatablished  ( 57) .	bind
18178	1	5720	6	NULL	NULL	0	NULL	Src	NULL		does not bind	NULL		K295R		ATP	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_2_875_s_227	14701758	(iii) Src(K295R) cannot bind ATP and has no basal or agonist activity.	bind
18179	2	5720	6	NULL	NULL	0	NULL	Src	NULL		does not exhibit	NULL		K295R		basal activity	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_2_875_s_227	14701758	(iii) Src(K295R) cannot bind ATP and has no basal or agonist activity.	bind
18180	3	5720	6	NULL	NULL	0	NULL	Src	NULL		does not exhibit	NULL		K295R		agonist activity	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_2_875_s_227	14701758	(iii) Src(K295R) cannot bind ATP and has no basal or agonist activity.	bind
17420	1	5720	7	NULL	NULL	NULL	NULL	Src	GP		does not bind			K295R		ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_2_875_s_227	14701758	(iii) Src(K295R) cannot bind ATP and has no basal or agonist activity.	bind
17421	2	5720	7	NULL	NULL	NULL	NULL	Src	GP		does not have			K295R		basal activity	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_2_875_s_227	14701758	(iii) Src(K295R) cannot bind ATP and has no basal or agonist activity.	bind
17422	3	5720	7	NULL	NULL	NULL	NULL	Src	GP		does not have			K295R		agonist activity	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_2_875_s_227	14701758	(iii) Src(K295R) cannot bind ATP and has no basal or agonist activity.	bind
18181	1	5721	6	NULL	NULL	0	NULL	LBP	NULL		bind	NULL		amino-terminal fragment		LPS	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_30_17934_s_128	7543094	(iii) The amino-terminal fragment of  LBP (residues 1-197) retains the LPS binding activity of the  native molecule( 15 ) .	bind
24956	1	5721	7	NULL	NULL	NULL	NULL	LBP	GP		binds			amino-terminal fragment		LPS	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_30_17934_s_128	7543094	(iii) The amino-terminal fragment of  LBP (residues 1-197) retains the LPS binding activity of the  native molecule( 15 ) .	bind
18182	1	5722	6	NULL	NULL	0	NULL	HRI	NULL	transformed	reassociates with	NULL				heme	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_5861_s_358	10454533	(iii) The binding of Hsc70 to transformed HRI which has reassociated with heme may facilitate a conformational change in HRI that is required for heme-induced inhibition of HRI activity (Fig.  10B,  3).	bind
18183	2	5722	6	NULL	NULL	0	NULL	Hsc70	NULL		bind	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_5861_s_358	10454533	(iii) The binding of Hsc70 to transformed HRI which has reassociated with heme may facilitate a conformational change in HRI that is required for heme-induced inhibition of HRI activity (Fig.  10B,  3).	bind
18184	3	5722	6	10	NULL	0	NULL	statement 2	NULL		facilitate	NULL	may			HRI	NULL	conformational change of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_5861_s_358	10454533	(iii) The binding of Hsc70 to transformed HRI which has reassociated with heme may facilitate a conformational change in HRI that is required for heme-induced inhibition of HRI activity (Fig.  10B,  3).	bind
18185	4	5722	6	NULL	NULL	0	NULL	heme	NULL		induce	NULL				HRI	NULL	inhibition of activity of 			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_5861_s_358	10454533	(iii) The binding of Hsc70 to transformed HRI which has reassociated with heme may facilitate a conformational change in HRI that is required for heme-induced inhibition of HRI activity (Fig.  10B,  3).	bind
23091	5	5722	6	NULL	NULL	0	NULL	statement 3	NULL		is required for	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_5861_s_358	10454533	(iii) The binding of Hsc70 to transformed HRI which has reassociated with heme may facilitate a conformational change in HRI that is required for heme-induced inhibition of HRI activity (Fig.  10B,  3).	bind
17424	2	5722	7	NULL	NULL	NULL	NULL	Hsc70	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_5861_s_358	10454533	(iii) The binding of Hsc70 to transformed HRI which has reassociated with heme may facilitate a conformational change in HRI that is required for heme-induced inhibition of HRI activity (Fig.  10B,  3).	bind
17425	1	5722	7	NULL	NULL	NULL	NULL	HRI	GP	transformed	reassociate with					heme	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_5861_s_358	10454533	(iii) The binding of Hsc70 to transformed HRI which has reassociated with heme may facilitate a conformational change in HRI that is required for heme-induced inhibition of HRI activity (Fig.  10B,  3).	bind
17426	3	5722	7	NULL	NULL	NULL	NULL	statement 2	Process		facilitate					HRI 	GP	conformational change in			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_5861_s_358	10454533	(iii) The binding of Hsc70 to transformed HRI which has reassociated with heme may facilitate a conformational change in HRI that is required for heme-induced inhibition of HRI activity (Fig.  10B,  3).	bind
17427	4	5722	7	NULL	NULL	NULL	NULL	heme	Chemical		induce					HRI	GP	inhibition of activity of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_5861_s_358	10454533	(iii) The binding of Hsc70 to transformed HRI which has reassociated with heme may facilitate a conformational change in HRI that is required for heme-induced inhibition of HRI activity (Fig.  10B,  3).	bind
17428	5	5722	7	NULL	NULL	NULL	NULL	statement 3	Process		is required for					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_5861_s_358	10454533	(iii) The binding of Hsc70 to transformed HRI which has reassociated with heme may facilitate a conformational change in HRI that is required for heme-induced inhibition of HRI activity (Fig.  10B,  3).	bind
18186	1	5723	6	NULL	NULL	0	NULL	IRS-2	NULL		interact with	NULL	specifically	amino acids 591 - 786		IR	NULL		KRLB of the beta subunit		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_15_14536_s_280	15705592	(iii) The IRS-2 sequence contains a unique region (amino acids 591 - 786), not present in IRS-1, which interacts specifically with the kinase regulatory loop binding (KRLB) domain of the beta-subunit of IR. (iv) There is a difference in the phosphorylation patterns of IRS-1 and IRS-2.	bind
18187	2	5723	6	NULL	NULL	0	NULL	KRLB	NULL		is	NULL				kinase regulatory loop binding	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_15_14536_s_280	15705592	(iii) The IRS-2 sequence contains a unique region (amino acids 591 - 786), not present in IRS-1, which interacts specifically with the kinase regulatory loop binding (KRLB) domain of the beta-subunit of IR. (iv) There is a difference in the phosphorylation patterns of IRS-1 and IRS-2.	bind
23092	3	5723	6	NULL	NULL	0	NULL	IRS-2	NULL		is not present in	NULL		amino acids 591-786		IRS-1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_15_14536_s_280	15705592	(iii) The IRS-2 sequence contains a unique region (amino acids 591 - 786), not present in IRS-1, which interacts specifically with the kinase regulatory loop binding (KRLB) domain of the beta-subunit of IR. (iv) There is a difference in the phosphorylation patterns of IRS-1 and IRS-2.	bind
23093	4	5723	6	NULL	NULL	0	NULL	IRS-1	NULL	phosphorylation pattern of	differs from	NULL				IRS-2	NULL	phosphorylation pattern of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_15_14536_s_280	15705592	(iii) The IRS-2 sequence contains a unique region (amino acids 591 - 786), not present in IRS-1, which interacts specifically with the kinase regulatory loop binding (KRLB) domain of the beta-subunit of IR. (iv) There is a difference in the phosphorylation patterns of IRS-1 and IRS-2.	bind
17429	1	5723	7	NULL	NULL	NULL	NULL	IRS-2	GP		binds		specifically	amino acids 591 - 786		IR	GP		KRLB of the beta subunit		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_15_14536_s_280	15705592	(iii) The IRS-2 sequence contains a unique region (amino acids 591 - 786), not present in IRS-1, which interacts specifically with the kinase regulatory loop binding (KRLB) domain of the beta-subunit of IR. (iv) There is a difference in the phosphorylation patterns of IRS-1 and IRS-2.	bind
17430	2	5723	7	NULL	NULL	NULL	NULL	KRLB	GP		is					kinase regulatory loop binding domain	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_15_14536_s_280	15705592	(iii) The IRS-2 sequence contains a unique region (amino acids 591 - 786), not present in IRS-1, which interacts specifically with the kinase regulatory loop binding (KRLB) domain of the beta-subunit of IR. (iv) There is a difference in the phosphorylation patterns of IRS-1 and IRS-2.	bind
17432	3	5723	7	NULL	NULL	NULL	NULL	IRS-2	GP	unique region	is not present in			 amino acids 591 - 786		IRS-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_15_14536_s_280	15705592	(iii) The IRS-2 sequence contains a unique region (amino acids 591 - 786), not present in IRS-1, which interacts specifically with the kinase regulatory loop binding (KRLB) domain of the beta-subunit of IR. (iv) There is a difference in the phosphorylation patterns of IRS-1 and IRS-2.	bind
17433	4	5723	7	NULL	NULL	NULL	NULL	IRS-1	GP	phosphorylation pattern of	differs from					IRS-2	GP	phosphorylation pattern of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_15_14536_s_280	15705592	(iii) The IRS-2 sequence contains a unique region (amino acids 591 - 786), not present in IRS-1, which interacts specifically with the kinase regulatory loop binding (KRLB) domain of the beta-subunit of IR. (iv) There is a difference in the phosphorylation patterns of IRS-1 and IRS-2.	bind
18188	1	5725	6	NULL	NULL	0	NULL	Fyn	NULL		bind	NULL		SH2 domain		tr-kit	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_embo_21_20_5386_s_186	12374739	(iii) The SH2 domain of Fyn, which binds  in vitro to tr-kit, or the Src-like kinase inhibitor PP2, suppress tr-kit-induced egg activation.	bind
18189	2	5725	6	10	NULL	0	NULL	Fyn	NULL		bind	NULL		SH2 domain		PP2	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_21_20_5386_s_186	12374739	(iii) The SH2 domain of Fyn, which binds  in vitro to tr-kit, or the Src-like kinase inhibitor PP2, suppress tr-kit-induced egg activation.	bind
18190	3	5725	6	NULL	NULL	0	NULL	tr-kit	NULL		induce	NULL				egg	NULL	activation of			NULL		NULL	NULL	NULL	NULL	gw60_embo_21_20_5386_s_186	12374739	(iii) The SH2 domain of Fyn, which binds  in vitro to tr-kit, or the Src-like kinase inhibitor PP2, suppress tr-kit-induced egg activation.	bind
18191	4	5725	6	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_21_20_5386_s_186	12374739	(iii) The SH2 domain of Fyn, which binds  in vitro to tr-kit, or the Src-like kinase inhibitor PP2, suppress tr-kit-induced egg activation.	bind
24586	5	5725	6	NULL	NULL	0	NULL	Fyn	NULL		suppress	NULL		SH2 domain		statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_21_20_5386_s_186	12374739	(iii) The SH2 domain of Fyn, which binds  in vitro to tr-kit, or the Src-like kinase inhibitor PP2, suppress tr-kit-induced egg activation.	bind
24587	6	5725	6	NULL	NULL	0	NULL	PP2	NULL		is a type of	NULL				Src-like kinase inhibitor	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_21_20_5386_s_186	12374739	(iii) The SH2 domain of Fyn, which binds  in vitro to tr-kit, or the Src-like kinase inhibitor PP2, suppress tr-kit-induced egg activation.	bind
17437	1	5725	7	NULL	NULL	NULL	NULL	Fyn	GP		binds			SH2 domain		tr-kit	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_21_20_5386_s_186	12374739	(iii) The SH2 domain of Fyn, which binds  in vitro to tr-kit, or the Src-like kinase inhibitor PP2, suppress tr-kit-induced egg activation.	bind
17438	2	5725	7	NULL	NULL	NULL	NULL	Fyn	GP		binds			SH2 domain		PP2	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_21_20_5386_s_186	12374739	(iii) The SH2 domain of Fyn, which binds  in vitro to tr-kit, or the Src-like kinase inhibitor PP2, suppress tr-kit-induced egg activation.	bind
17439	3	5725	7	NULL	NULL	NULL	NULL	PP2	GP		is a type of 					Src-like kinase inhibitor	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_20_5386_s_186	12374739	(iii) The SH2 domain of Fyn, which binds  in vitro to tr-kit, or the Src-like kinase inhibitor PP2, suppress tr-kit-induced egg activation.	bind
17440	4	5725	7	NULL	NULL	NULL	NULL	tr-kit	GP		induce					egg	Organism	activation of			NULL		NULL	NULL	NULL	NULL	gw60_embo_21_20_5386_s_186	12374739	(iii) The SH2 domain of Fyn, which binds  in vitro to tr-kit, or the Src-like kinase inhibitor PP2, suppress tr-kit-induced egg activation.	bind
17441	5	5725	7	NULL	NULL	NULL	NULL	Fyn	GP		suppress			SH2 domain		statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_20_5386_s_186	12374739	(iii) The SH2 domain of Fyn, which binds  in vitro to tr-kit, or the Src-like kinase inhibitor PP2, suppress tr-kit-induced egg activation.	bind
24957	6	5725	7	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_20_5386_s_186	12374739	(iii) The SH2 domain of Fyn, which binds  in vitro to tr-kit, or the Src-like kinase inhibitor PP2, suppress tr-kit-induced egg activation.	bind
18192	1	5726	6	NULL	NULL	0	NULL	Rb+	NULL		bind	NULL				E1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_8_5910_s_374	11739377	(iii) The very large values of the constants of the reactions that lead to occlusion after the binding of Rb+ to  E1 are not enough to explain the time-independent component of the occlusion curves.	bind
17442	1	5726	7	NULL	NULL	NULL	NULL	Rb+	Chemical		bind					E1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_8_5910_s_374	11739377	(iii) The very large values of the constants of the reactions that lead to occlusion after the binding of Rb+ to  E1 are not enough to explain the time-independent component of the occlusion curves.	bind
18193	1	5727	6	10	NULL	0	NULL	UV-DDB	NULL		bind	NULL	high affinity;;specifically			DNA	NULL	UV-irradiated			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9784_s_192	16260596	(iii) UV-DDB binds to UV-irradiated DNA ( ,  ) and in particular to (6-4) photoproducts ( ) with high affinity and specificity.	bind
18194	2	5727	6	NULL	NULL	0	NULL	UV-DDB	NULL		bind	NULL	high affinity;;specifically			photoproducts	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9784_s_192	16260596	(iii) UV-DDB binds to UV-irradiated DNA ( ,  ) and in particular to (6-4) photoproducts ( ) with high affinity and specificity.	bind
17443	1	5727	7	NULL	NULL	NULL	NULL	UV-DDB	GP		binds		high affinity;;specifically			DNA	NucleicAcid	UV-irradiated			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9784_s_192	16260596	(iii) UV-DDB binds to UV-irradiated DNA ( ,  ) and in particular to (6-4) photoproducts ( ) with high affinity and specificity.	bind
17444	2	5727	7	NULL	NULL	NULL	NULL	UV-DDB	GP		binds		high affinity;;specifically			photoproducts	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9784_s_192	16260596	(iii) UV-DDB binds to UV-irradiated DNA ( ,  ) and in particular to (6-4) photoproducts ( ) with high affinity and specificity.	bind
18195	1	5728	6	NULL	NULL	0	NULL	Mdm2	NULL	wild type	bind	NULL				p14ARF	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6170_s_244	12167711	(iii) Wild-type and mutant Mdm2 bind to p14ARF with equal affinities.	bind
18196	2	5728	6	NULL	NULL	0	NULL	Mdm2	NULL	mutant	bind	NULL				p14ARF	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6170_s_244	12167711	(iii) Wild-type and mutant Mdm2 bind to p14ARF with equal affinities.	bind
18197	3	5728	6	NULL	NULL	0	NULL	statement 1	NULL	affinity of	is equal to	NULL				statement 2	NULL	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6170_s_244	12167711	(iii) Wild-type and mutant Mdm2 bind to p14ARF with equal affinities.	bind
17447	1	5728	7	NULL	NULL	NULL	NULL	Mdm2	GP	Wild-type	bind					p14ARF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6170_s_244	12167711	(iii) Wild-type and mutant Mdm2 bind to p14ARF with equal affinities.	bind
17448	2	5728	7	NULL	NULL	NULL	NULL	Mdm2	GP	mutant	bind					p14 ARF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6170_s_244	12167711	(iii) Wild-type and mutant Mdm2 bind to p14ARF with equal affinities.	bind
17449	3	5728	7	NULL	NULL	NULL	NULL	statement 1	Process	affinity of	is equal to					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6170_s_244	12167711	(iii) Wild-type and mutant Mdm2 bind to p14ARF with equal affinities.	bind
18198	1	5729	6	10	NULL	0	NULL	AMP	NULL		bind	NULL					NULL		ATP-BD		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_3_2234_s_203	11053407	(In fact, AMP consistently produced a small increase in the fluorescence of the ATP-pretreated sample, further illustrating that AMP was bound to ATP-BD, but did not compete with TNP-ATP.)	bind
18204	2	5729	6	10	NULL	0	NULL	TNP	NULL		bind	NULL					NULL		ATP-BD		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_3_2234_s_203	11053407	(In fact, AMP consistently produced a small increase in the fluorescence of the ATP-pretreated sample, further illustrating that AMP was bound to ATP-BD, but did not compete with TNP-ATP.)	bind
18205	3	5729	6	10	NULL	0	NULL	statement 1	NULL		does not compete	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_3_2234_s_203	11053407	(In fact, AMP consistently produced a small increase in the fluorescence of the ATP-pretreated sample, further illustrating that AMP was bound to ATP-BD, but did not compete with TNP-ATP.)	bind
17450	1	5729	7	NULL	NULL	NULL	NULL	AMP	Chemical		bind								ATP-BD		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_3_2234_s_203	11053407	(In fact, AMP consistently produced a small increase in the fluorescence of the ATP-pretreated sample, further illustrating that AMP was bound to ATP-BD, but did not compete with TNP-ATP.)	bind
17451	2	5729	7	NULL	NULL	NULL	NULL	TNP	Chemical		bind								ATP-BD		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_3_2234_s_203	11053407	(In fact, AMP consistently produced a small increase in the fluorescence of the ATP-pretreated sample, further illustrating that AMP was bound to ATP-BD, but did not compete with TNP-ATP.)	bind
17452	3	5729	7	NULL	NULL	NULL	NULL	statement 1	Process		does not compete with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_3_2234_s_203	11053407	(In fact, AMP consistently produced a small increase in the fluorescence of the ATP-pretreated sample, further illustrating that AMP was bound to ATP-BD, but did not compete with TNP-ATP.)	bind
18206	1	5730	6	10	NULL	0	NULL	anti-human Fc	NULL		stabilizes	NULL	significantly			Ntm-Fc	NULL	binding of 			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_18_22_9312_s_213	9801370	(In other studies, we found that cross-linking with the anti-human Fc significantly stabilized the binding of the Ntm-Fc; data not shown.)	bind
17455	1	5730	7	NULL	NULL	NULL	NULL	anti-human Fc	GP		stabilize		significantly			Ntm-Fc	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_18_22_9312_s_213	9801370	(In other studies, we found that cross-linking with the anti-human Fc significantly stabilized the binding of the Ntm-Fc; data not shown.)	bind
18207	1	5732	6	10	NULL	0	NULL	Ddi1	NULL		lacks	NULL					NULL		UbA domain		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_5_1579_s_278	16478980	(In this scenario one possible explanation for the marked reduction [ca. 90% in the binding of Ufo1 to Ddi1 lacking its UbA domain may reflect a similar lack of accessibility to the Ddi1 core.)	bind
45756	2	5732	6	10	NULL	0	NULL	Ufo1	NULL		bind	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_5_1579_s_278	16478980	(In this scenario one possible explanation for the marked reduction [ca. 90% in the binding of Ufo1 to Ddi1 lacking its UbA domain may reflect a similar lack of accessibility to the Ddi1 core.)	bind
17456	2	5732	7	NULL	NULL	NULL	NULL	Ufo1	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_5_1579_s_278	16478980	(In this scenario one possible explanation for the marked reduction [ca. 90% in the binding of Ufo1 to Ddi1 lacking its UbA domain may reflect a similar lack of accessibility to the Ddi1 core.)	bind
17457	1	5732	7	NULL	NULL	NULL	NULL	Ddi1	GP		lacks								UbA domain		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_5_1579_s_278	16478980	(In this scenario one possible explanation for the marked reduction [ca. 90% in the binding of Ufo1 to Ddi1 lacking its UbA domain may reflect a similar lack of accessibility to the Ddi1 core.)	bind
18208	1	5733	6	NULL	NULL	0	NULL	RAG1	NULL		is limited to	NULL		importin alpha binding site		importin alpha1	NULL		98-amino acid fragment		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_22_16752_s_220	10748034	(In unpublished data described in Ref.  48, the importin alpha binding site of RAG1 was limited to the same 98-amino acid fragment of importin alpha1 that we identified (432-529).)	bind
17817	1	5733	7	NULL	NULL	NULL	NULL	RAG1	GP		is limited to			importin alpha binding site of		importin alpha1	GP		98-amino acid fragment		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_22_16752_s_220	10748034	(In unpublished data described in Ref.  48, the importin alpha binding site of RAG1 was limited to the same 98-amino acid fragment of importin alpha1 that we identified (432-529).)	bind
18210	1	5734	6	10	NULL	0	NULL	TC-[57Co]Cbl complex	NULL		bind	NULL				HMEC	NULL				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1528_1_43_s_106	11514097	(Inset) Analysis of TC-[57Co]Cbl complex binding to HMEC.	bind
17458	1	5734	7	NULL	NULL	NULL	NULL	TC-[57Co]Cbl complex 	Chemical		bind					HMEC	Cell				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1528_1_43_s_106	11514097	(Inset) Analysis of TC-[57Co]Cbl complex binding to HMEC.	bind
18211	1	5736	6	NULL	NULL	0	NULL	Streptokinase	NULL		bind	NULL				plasminogen	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_71_4_1903_s_169	12654807	(Interaction 3) Streptokinase binds plasminogen and GAS M protein binds fibrinogen.	bind
18212	2	5736	6	NULL	NULL	0	NULL	GAS M protein	NULL		bind	NULL				fibrinogen	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_71_4_1903_s_169	12654807	(Interaction 3) Streptokinase binds plasminogen and GAS M protein binds fibrinogen.	bind
17459	1	5736	7	NULL	NULL	NULL	NULL	Streptokinase	GP		binds					plasminogen	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_71_4_1903_s_169	12654807	(Interaction 3) Streptokinase binds plasminogen and GAS M protein binds fibrinogen.	bind
17460	2	5736	7	NULL	NULL	NULL	NULL	GAS M protein	GP		binds					fibrinogen	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_71_4_1903_s_169	12654807	(Interaction 3) Streptokinase binds plasminogen and GAS M protein binds fibrinogen.	bind
18213	1	5739	6	NULL	NULL	0	NULL	Mei4 protein	NULL	recombinant	bind	NULL	specifically			spo6+	NULL			FLEX-D DNA fragment	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_4_2118_s_360	9528784	(iv) A recombinant Mei4 protein could bind specifically to the FLEX-D DNA fragment, a putative  cis element on  spo6+.	bind
53246	2	5739	6	10	NULL	0	NULL	FLEX-D DNA fragment	NULL		is a type of	NULL				putative cis element on spo6+	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_4_2118_s_360	9528784	(iv) A recombinant Mei4 protein could bind specifically to the FLEX-D DNA fragment, a putative  cis element on  spo6+.	bind
17461	1	5739	7	10	NULL	0	NULL	Mei4 protein	NULL	recombinant	bind	NULL	specifically			spo6	NULL			FLEX-D DNA fragment	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2118_s_360	9528784	(iv) A recombinant Mei4 protein could bind specifically to the FLEX-D DNA fragment, a putative  cis element on  spo6+.	bind
17462	2	5739	7	10	NULL	0	NULL	FLEX-D DNA fragment	NULL		is a type of	NULL				putative cis element on spo6+	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2118_s_360	9528784	(iv) A recombinant Mei4 protein could bind specifically to the FLEX-D DNA fragment, a putative  cis element on  spo6+.	bind
18214	1	5740	6	NULL	NULL	0	NULL	MyoD	NULL		bind	NULL				DNA	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_12	11940648	(iv) Addition of p204 overcame the inhibition by the Id proteins of the binding of MyoD and E47 to DNA in vitro.	bind
18215	2	5740	6	NULL	NULL	0	NULL	E47	NULL		bind	NULL				DNA	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_12	11940648	(iv) Addition of p204 overcame the inhibition by the Id proteins of the binding of MyoD and E47 to DNA in vitro.	bind
18216	3	5740	6	10	NULL	0	NULL	Id protein	NULL		inhibit	NULL				statement 1	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_12	11940648	(iv) Addition of p204 overcame the inhibition by the Id proteins of the binding of MyoD and E47 to DNA in vitro.	bind
18217	4	5740	6	10	NULL	0	NULL	Id protein	NULL		inhibit	NULL				statement 2	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_12	11940648	(iv) Addition of p204 overcame the inhibition by the Id proteins of the binding of MyoD and E47 to DNA in vitro.	bind
18308	5	5740	6	10	NULL	0	NULL	p204	NULL		overcome	NULL				statement 3	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_12	11940648	(iv) Addition of p204 overcame the inhibition by the Id proteins of the binding of MyoD and E47 to DNA in vitro.	bind
18309	6	5740	6	10	NULL	0	NULL	p204	NULL		overcome	NULL				statement 4	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_12	11940648	(iv) Addition of p204 overcame the inhibition by the Id proteins of the binding of MyoD and E47 to DNA in vitro.	bind
17463	1	5740	7	NULL	NULL	NULL	NULL	MyoD	GP		binds					DNA	NucleicAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_12	11940648	(iv) Addition of p204 overcame the inhibition by the Id proteins of the binding of MyoD and E47 to DNA in vitro.	bind
17464	2	5740	7	NULL	NULL	NULL	NULL	E47	GP		binds					DNA	NucleicAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_12	11940648	(iv) Addition of p204 overcame the inhibition by the Id proteins of the binding of MyoD and E47 to DNA in vitro.	bind
17465	3	5740	7	NULL	NULL	NULL	NULL	Id proteins	Gp		inhibits					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_12	11940648	(iv) Addition of p204 overcame the inhibition by the Id proteins of the binding of MyoD and E47 to DNA in vitro.	bind
17466	4	5740	7	NULL	NULL	NULL	NULL	Id proteins	GP		inhibits					statement 2	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_12	11940648	(iv) Addition of p204 overcame the inhibition by the Id proteins of the binding of MyoD and E47 to DNA in vitro.	bind
17467	5	5740	7	NULL	NULL	NULL	NULL	p204	GP	addition of	overcame					statement 3	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_12	11940648	(iv) Addition of p204 overcame the inhibition by the Id proteins of the binding of MyoD and E47 to DNA in vitro.	bind
17468	6	5740	7	NULL	NULL	NULL	NULL	p204	GP	addition of	overcame					statement 4	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_9_2893_s_12	11940648	(iv) Addition of p204 overcame the inhibition by the Id proteins of the binding of MyoD and E47 to DNA in vitro.	bind
18310	1	5741	6	NULL	NULL	0	NULL	Tim17	NULL		bind	NULL				mtHsp70	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_16_9_2205_s_69	9171336	(iv) As a further control to exclude a post-lysis binding of Tim17 or Tim23 to mtHsp70, the Tim proteins were imported into  ssc1-3 mitochondria, where they were correctly integrated into the inner membrane but did not bind to the mutant Hsp70 (Figure  2D, lane 6).	bind
18311	2	5741	6	NULL	NULL	0	NULL	Tim23	NULL		bind	NULL				mtHsp70	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_16_9_2205_s_69	9171336	(iv) As a further control to exclude a post-lysis binding of Tim17 or Tim23 to mtHsp70, the Tim proteins were imported into  ssc1-3 mitochondria, where they were correctly integrated into the inner membrane but did not bind to the mutant Hsp70 (Figure  2D, lane 6).	bind
18312	3	5741	6	NULL	NULL	0	NULL	Tim proteins	NULL		imported into	NULL				ssc1-3 mitochondria	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_16_9_2205_s_69	9171336	(iv) As a further control to exclude a post-lysis binding of Tim17 or Tim23 to mtHsp70, the Tim proteins were imported into  ssc1-3 mitochondria, where they were correctly integrated into the inner membrane but did not bind to the mutant Hsp70 (Figure  2D, lane 6).	bind
18313	4	5741	6	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_16_9_2205_s_69	9171336	(iv) As a further control to exclude a post-lysis binding of Tim17 or Tim23 to mtHsp70, the Tim proteins were imported into  ssc1-3 mitochondria, where they were correctly integrated into the inner membrane but did not bind to the mutant Hsp70 (Figure  2D, lane 6).	bind
18314	5	5741	6	NULL	NULL	0	NULL	Tim proteins	NULL		does not bind	NULL				Hsp70	NULL	mutant			NULL		0	NULL	NULL	NULL	gw60_embo_16_9_2205_s_69	9171336	(iv) As a further control to exclude a post-lysis binding of Tim17 or Tim23 to mtHsp70, the Tim proteins were imported into  ssc1-3 mitochondria, where they were correctly integrated into the inner membrane but did not bind to the mutant Hsp70 (Figure  2D, lane 6).	bind
45759	6	5741	6	10	NULL	0	NULL	statement 3	NULL		is integrated into	NULL				inner membrane	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_16_9_2205_s_69	9171336	(iv) As a further control to exclude a post-lysis binding of Tim17 or Tim23 to mtHsp70, the Tim proteins were imported into  ssc1-3 mitochondria, where they were correctly integrated into the inner membrane but did not bind to the mutant Hsp70 (Figure  2D, lane 6).	bind
17469	3	5741	7	NULL	NULL	NULL	NULL	Tim proteins	GP		imported to					 ssc1-3 mitochondria	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_9_2205_s_69	9171336	(iv) As a further control to exclude a post-lysis binding of Tim17 or Tim23 to mtHsp70, the Tim proteins were imported into  ssc1-3 mitochondria, where they were correctly integrated into the inner membrane but did not bind to the mutant Hsp70 (Figure  2D, lane 6).	bind
17470	4	5741	7	NULL	NULL	NULL	NULL	statement 1	Process		 integrated to		correctly			inner membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_9_2205_s_69	9171336	(iv) As a further control to exclude a post-lysis binding of Tim17 or Tim23 to mtHsp70, the Tim proteins were imported into  ssc1-3 mitochondria, where they were correctly integrated into the inner membrane but did not bind to the mutant Hsp70 (Figure  2D, lane 6).	bind
17471	5	5741	7	NULL	NULL	NULL	NULL	Tim proteins	GP		does not bind					Hsp70	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_embo_16_9_2205_s_69	9171336	(iv) As a further control to exclude a post-lysis binding of Tim17 or Tim23 to mtHsp70, the Tim proteins were imported into  ssc1-3 mitochondria, where they were correctly integrated into the inner membrane but did not bind to the mutant Hsp70 (Figure  2D, lane 6).	bind
45853	1	5741	7	NULL	NULL	NULL	NULL	Tim17	GP		bind					mtHsp70	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_9_2205_s_69	9171336	(iv) As a further control to exclude a post-lysis binding of Tim17 or Tim23 to mtHsp70, the Tim proteins were imported into  ssc1-3 mitochondria, where they were correctly integrated into the inner membrane but did not bind to the mutant Hsp70 (Figure  2D, lane 6).	bind
45854	2	5741	7	NULL	NULL	NULL	NULL	Tim23	GP		bind					mtHsp70	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_9_2205_s_69	9171336	(iv) As a further control to exclude a post-lysis binding of Tim17 or Tim23 to mtHsp70, the Tim proteins were imported into  ssc1-3 mitochondria, where they were correctly integrated into the inner membrane but did not bind to the mutant Hsp70 (Figure  2D, lane 6).	bind
45855	6	5741	7	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_9_2205_s_69	9171336	(iv) As a further control to exclude a post-lysis binding of Tim17 or Tim23 to mtHsp70, the Tim proteins were imported into  ssc1-3 mitochondria, where they were correctly integrated into the inner membrane but did not bind to the mutant Hsp70 (Figure  2D, lane 6).	bind
18315	1	5742	6	NULL	NULL	0	NULL	myosin	NULL		bind	NULL	strongly			actin	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_19_6873_s_23	15863618	(IV) ATP hydrolysis remains reversible until myosin binds strongly  to actin ( ).	bind
18316	2	5742	6	NULL	NULL	0	NULL	ATP	NULL	hydrolysis of	is dependent on	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_19_6873_s_23	15863618	(IV) ATP hydrolysis remains reversible until myosin binds strongly  to actin ( ).	bind
17472	1	5742	7	NULL	NULL	NULL	NULL	 myosin 	GP		binds		strongly			actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_19_6873_s_23	15863618	(IV) ATP hydrolysis remains reversible until myosin binds strongly  to actin ( ).	bind
17473	2	5742	7	NULL	NULL	NULL	NULL	ATP	Chemical	hydrolysis of	remains					reversible	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_19_6873_s_23	15863618	(IV) ATP hydrolysis remains reversible until myosin binds strongly  to actin ( ).	bind
17474	3	5742	7	NULL	NULL	NULL	NULL	statement 2	Process		happens until					statement 1	Process	occurance of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_19_6873_s_23	15863618	(IV) ATP hydrolysis remains reversible until myosin binds strongly  to actin ( ).	bind
18317	1	5743	6	NULL	NULL	0	NULL	Msb3	NULL		bind	NULL				Rho GTPase	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_19_8567_s_132	16166638	(iv) Binding of Msb3 and Msb4 to Rho GTPases.	bind
18318	2	5743	6	NULL	NULL	0	NULL	Msb4	NULL		bind	NULL				Rho GTPase	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_19_8567_s_132	16166638	(iv) Binding of Msb3 and Msb4 to Rho GTPases.	bind
17475	1	5743	7	NULL	NULL	NULL	NULL	Msb3	GP		bind					Rho GTPases	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8567_s_132	16166638	(iv) Binding of Msb3 and Msb4 to Rho GTPases.	bind
17476	2	5743	7	NULL	NULL	NULL	NULL	Msb4	GP		bind					Rho GTPases	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_19_8567_s_132	16166638	(iv) Binding of Msb3 and Msb4 to Rho GTPases.	bind
18463	1	5744	6	NULL	NULL	0	NULL	plasminogen	NULL	cell surface	activates into	NULL				plasmin	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_16_24_7279_s_92	9405357	(iv) Binding of uPA to uPAR/CD87 activates cell surface plasminogen to plasmin which also might cleave uPAR/CD87 in the same region (Hoyer-Hansen  et al., 1992  ; Ploug and Ellis, 1994  ).	bind
18464	2	5744	6	NULL	NULL	0	NULL	uPA	NULL		bind	NULL				uPAR/CD87	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_16_24_7279_s_92	9405357	(iv) Binding of uPA to uPAR/CD87 activates cell surface plasminogen to plasmin which also might cleave uPAR/CD87 in the same region (Hoyer-Hansen  et al., 1992  ; Ploug and Ellis, 1994  ).	bind
18465	3	5744	6	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_16_24_7279_s_92	9405357	(iv) Binding of uPA to uPAR/CD87 activates cell surface plasminogen to plasmin which also might cleave uPAR/CD87 in the same region (Hoyer-Hansen  et al., 1992  ; Ploug and Ellis, 1994  ).	bind
18466	4	5744	6	NULL	NULL	0	NULL	statement 1	NULL		cleave	NULL	may			uPAR/CD87 	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_16_24_7279_s_92	9405357	(iv) Binding of uPA to uPAR/CD87 activates cell surface plasminogen to plasmin which also might cleave uPAR/CD87 in the same region (Hoyer-Hansen  et al., 1992  ; Ploug and Ellis, 1994  ).	bind
17477	1	5744	7	NULL	NULL	NULL	NULL	uPA	GP		bind					uPAR/CD87	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_24_7279_s_92	9405357	(iv) Binding of uPA to uPAR/CD87 activates cell surface plasminogen to plasmin which also might cleave uPAR/CD87 in the same region (Hoyer-Hansen  et al., 1992  ; Ploug and Ellis, 1994  ).	bind
17478	2	5744	7	NULL	NULL	NULL	NULL	plasminogen	GP	cell surface	converts to					plasmin	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_24_7279_s_92	9405357	(iv) Binding of uPA to uPAR/CD87 activates cell surface plasminogen to plasmin which also might cleave uPAR/CD87 in the same region (Hoyer-Hansen  et al., 1992  ; Ploug and Ellis, 1994  ).	bind
17479	3	5744	7	NULL	NULL	NULL	NULL	statement 1	Process		activates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_24_7279_s_92	9405357	(iv) Binding of uPA to uPAR/CD87 activates cell surface plasminogen to plasmin which also might cleave uPAR/CD87 in the same region (Hoyer-Hansen  et al., 1992  ; Ploug and Ellis, 1994  ).	bind
17480	4	5744	7	NULL	NULL	NULL	NULL	plasmin	GP		cleave					uPAR/CD87	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_24_7279_s_92	9405357	(iv) Binding of uPA to uPAR/CD87 activates cell surface plasminogen to plasmin which also might cleave uPAR/CD87 in the same region (Hoyer-Hansen  et al., 1992  ; Ploug and Ellis, 1994  ).	bind
18319	1	5745	6	NULL	NULL	0	NULL	P22	NULL		bind	NULL				LDC	NULL	S.ruminantium			NULL		0	NULL	NULL	NULL	abs-batch0600-0619_j-biol-chem_281_7_16354653_s_11	16354653	(iv) Both P22 and mouse AZ bind to S. ruminantium  LDC but not to the LDC mutated in its binding site for P22 and AZ.	bind
18320	2	5745	6	NULL	NULL	0	NULL	AZ	NULL	mouse	bind	NULL				LDC	NULL	S.ruminantium			NULL		0	NULL	NULL	NULL	abs-batch0600-0619_j-biol-chem_281_7_16354653_s_11	16354653	(iv) Both P22 and mouse AZ bind to S. ruminantium  LDC but not to the LDC mutated in its binding site for P22 and AZ.	bind
18321	3	5745	6	NULL	NULL	0	NULL	P22	NULL		does not bind	NULL				LDC	NULL	mutant S.ruminantium	p22 binding site		NULL		0	NULL	NULL	NULL	abs-batch0600-0619_j-biol-chem_281_7_16354653_s_11	16354653	(iv) Both P22 and mouse AZ bind to S. ruminantium  LDC but not to the LDC mutated in its binding site for P22 and AZ.	bind
18322	4	5745	6	NULL	NULL	0	NULL	AZ	NULL	mouse	does not bind	NULL				LDC	NULL	mutant S.ruminantium	AZ binding site		NULL		0	NULL	NULL	NULL	abs-batch0600-0619_j-biol-chem_281_7_16354653_s_11	16354653	(iv) Both P22 and mouse AZ bind to S. ruminantium  LDC but not to the LDC mutated in its binding site for P22 and AZ.	bind
17482	1	5745	7	NULL	NULL	NULL	NULL	P22	GP		bind					LDC	GP	S. ruminantium 			NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_j-biol-chem_281_7_16354653_s_11	16354653	(iv) Both P22 and mouse AZ bind to S. ruminantium  LDC but not to the LDC mutated in its binding site for P22 and AZ.	bind
17483	2	5745	7	NULL	NULL	NULL	NULL	AZ	GP	mouse	bind					LDC	GP	S. ruminantium 			NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_j-biol-chem_281_7_16354653_s_11	16354653	(iv) Both P22 and mouse AZ bind to S. ruminantium  LDC but not to the LDC mutated in its binding site for P22 and AZ.	bind
17484	3	5745	7	NULL	NULL	NULL	NULL	P22	GP		does not bind					LDC	GP	S. ruminantium mutated at	P22 binding site		NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_j-biol-chem_281_7_16354653_s_11	16354653	(iv) Both P22 and mouse AZ bind to S. ruminantium  LDC but not to the LDC mutated in its binding site for P22 and AZ.	bind
17485	4	5745	7	NULL	NULL	NULL	NULL	AZ	GP		does not bind					LDC	GP	S. ruminantium mutated at	AZ binding site		NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_j-biol-chem_281_7_16354653_s_11	16354653	(iv) Both P22 and mouse AZ bind to S. ruminantium  LDC but not to the LDC mutated in its binding site for P22 and AZ.	bind
18323	1	5746	6	NULL	NULL	0	NULL	Ca+2	NULL		bind	NULL				EGF-1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_28_17467_s_180	9211891	(iv) Ca2+ binding to EGF-1 does not affect the VIIa interaction with TF residue Gln110.	bind
18324	2	5746	6	NULL	NULL	0	NULL	VIIa	NULL		interacts with	NULL				TF residue Gln110	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_28_17467_s_180	9211891	(iv) Ca2+ binding to EGF-1 does not affect the VIIa interaction with TF residue Gln110.	bind
18325	3	5746	6	NULL	NULL	0	NULL	statement 1	NULL		does not affect	NULL	                                                                                                                            			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_28_17467_s_180	9211891	(iv) Ca2+ binding to EGF-1 does not affect the VIIa interaction with TF residue Gln110.	bind
17486	1	5746	7	NULL	NULL	NULL	NULL	Ca2+	Chemical		binds to					EGF-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17467_s_180	9211891	(iv) Ca2+ binding to EGF-1 does not affect the VIIa interaction with TF residue Gln110.	bind
17487	2	5746	7	NULL	NULL	NULL	NULL	 VIIa	GP		interacts with					TF residue Gln110	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17467_s_180	9211891	(iv) Ca2+ binding to EGF-1 does not affect the VIIa interaction with TF residue Gln110.	bind
17488	3	5746	7	NULL	NULL	NULL	NULL	statement 1	Process		does not affect					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17467_s_180	9211891	(iv) Ca2+ binding to EGF-1 does not affect the VIIa interaction with TF residue Gln110.	bind
18326	1	5747	6	10	NULL	0	NULL	fibronectin	NULL		bind	NULL				fibrinogen	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_j-thromb-haemost_3_8_16102057_s_12	16102057	(iv) Enhanced interactions with the extracellular matrix by  binding of fibronectin to fibrin(ogen).	bind
17532	1	5747	7	NULL	NULL	NULL	NULL	fibronectin	GP		binds					fibrinogen	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_j-thromb-haemost_3_8_16102057_s_12	16102057	(iv) Enhanced interactions with the extracellular matrix by  binding of fibronectin to fibrin(ogen).	bind
18327	1	5748	6	NULL	NULL	0	NULL	fatty acid	NULL		bind	NULL				FadL	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw70_microbiolmolbiolr_67_3_454_s_140	12966144	(iv) Fatty acid binding to FadL has been demonstrated both in vivo and in vitro ( ).	bind
18328	2	5748	6	NULL	NULL	0	NULL	fatty acid	NULL		bind	NULL				FadL	NULL				NULL	in vivo	0	NULL	NULL	NULL	gw70_microbiolmolbiolr_67_3_454_s_140	12966144	(iv) Fatty acid binding to FadL has been demonstrated both in vivo and in vitro ( ).	bind
17534	1	5748	7	NULL	NULL	NULL	NULL	Fatty acid	Chemical		bind					FadL	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_67_3_454_s_140	12966144	(iv) Fatty acid binding to FadL has been demonstrated both in vivo and in vitro ( ).	bind
17535	2	5748	7	NULL	NULL	NULL	NULL	Fatty acid	Chemical		bind					FadL	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_67_3_454_s_140	12966144	(iv) Fatty acid binding to FadL has been demonstrated both in vivo and in vitro ( ).	bind
18329	1	5751	6	NULL	NULL	0	NULL	GadX	NULL		bind	NULL	directly			gadW	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_23_6852_s_221	14617649	(iv) GadW is also acid induced by an unknown mechanism when it is not repressed by GadX. (v) GadX directly binds to the  gadW promoter region.	bind
18384	2	5751	6	NULL	NULL	0	NULL	GadW	NULL		is induced by	NULL				acid	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_23_6852_s_221	14617649	(iv) GadW is also acid induced by an unknown mechanism when it is not repressed by GadX. (v) GadX directly binds to the  gadW promoter region.	bind
18411	3	5751	6	NULL	NULL	0	NULL	GadX	NULL		represses	NULL				GadW	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_23_6852_s_221	14617649	(iv) GadW is also acid induced by an unknown mechanism when it is not repressed by GadX. (v) GadX directly binds to the  gadW promoter region.	bind
24585	4	5751	6	NULL	NULL	0	NULL	statement 2	NULL		occurs in absence of	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_23_6852_s_221	14617649	(iv) GadW is also acid induced by an unknown mechanism when it is not repressed by GadX. (v) GadX directly binds to the  gadW promoter region.	bind
17540	1	5751	7	NULL	NULL	NULL	NULL	acid	Chemical		induce					GadW	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_23_6852_s_221	14617649	(iv) GadW is also acid induced by an unknown mechanism when it is not repressed by GadX. (v) GadX directly binds to the  gadW promoter region.	bind
17541	2	5751	7	NULL	NULL	NULL	NULL	GadX	GP		repress					GadW	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_23_6852_s_221	14617649	(iv) GadW is also acid induced by an unknown mechanism when it is not repressed by GadX. (v) GadX directly binds to the  gadW promoter region.	bind
17542	3	5751	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs in the absence of					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_23_6852_s_221	14617649	(iv) GadW is also acid induced by an unknown mechanism when it is not repressed by GadX. (v) GadX directly binds to the  gadW promoter region.	bind
17543	4	5751	7	NULL	NULL	NULL	NULL	GadX	GP		binds		directly			gadW	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_23_6852_s_221	14617649	(iv) GadW is also acid induced by an unknown mechanism when it is not repressed by GadX. (v) GadX directly binds to the  gadW promoter region.	bind
18412	1	5752	6	NULL	NULL	0	NULL	leucine	NULL		bind	NULL				Sa-Lrp protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_13_3661_s_264	10850980	(iv) Most significantly, L-leucine specifically protects the archaeal Sa-Lrp binding capacity against irreversible heat inactivation; this effect likely reflects a physiologically significant interaction of leucine with the Sa-Lrp protein and suggests that leucine might function as the main effector of a hypothetical regulon.	bind
18413	2	5752	6	NULL	NULL	0	NULL	L-leucine	NULL		protects	NULL	specifically			Sa-Lrp	NULL	binding capacity of 			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_13_3661_s_264	10850980	(iv) Most significantly, L-leucine specifically protects the archaeal Sa-Lrp binding capacity against irreversible heat inactivation; this effect likely reflects a physiologically significant interaction of leucine with the Sa-Lrp protein and suggests that leucine might function as the main effector of a hypothetical regulon.	bind
18414	3	5752	6	10	NULL	0	NULL	statement 2	NULL		occurs against	NULL				heat inactivation	NULL	irreversible			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_13_3661_s_264	10850980	(iv) Most significantly, L-leucine specifically protects the archaeal Sa-Lrp binding capacity against irreversible heat inactivation; this effect likely reflects a physiologically significant interaction of leucine with the Sa-Lrp protein and suggests that leucine might function as the main effector of a hypothetical regulon.	bind
17544	1	5752	7	NULL	NULL	NULL	NULL	leucine	AminoAcid		binds					Sa-Lrp protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_13_3661_s_264	10850980	(iv) Most significantly, L-leucine specifically protects the archaeal Sa-Lrp binding capacity against irreversible heat inactivation; this effect likely reflects a physiologically significant interaction of leucine with the Sa-Lrp protein and suggests that leucine might function as the main effector of a hypothetical regulon.	bind
17545	2	5752	7	NULL	NULL	NULL	NULL	L-leucine	AminoAcid		protects		specifically			Sa-Lrp	GP	binding of archeal			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_13_3661_s_264	10850980	(iv) Most significantly, L-leucine specifically protects the archaeal Sa-Lrp binding capacity against irreversible heat inactivation; this effect likely reflects a physiologically significant interaction of leucine with the Sa-Lrp protein and suggests that leucine might function as the main effector of a hypothetical regulon.	bind
17546	3	5752	7	NULL	NULL	NULL	NULL	statement 2	Process		protects against					 heat inactivation	Process	irreversible			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_13_3661_s_264	10850980	(iv) Most significantly, L-leucine specifically protects the archaeal Sa-Lrp binding capacity against irreversible heat inactivation; this effect likely reflects a physiologically significant interaction of leucine with the Sa-Lrp protein and suggests that leucine might function as the main effector of a hypothetical regulon.	bind
17547	4	5752	7	NULL	NULL	NULL	NULL	leucine	AminoAcid		function as		might			regulon	GP	main effector of;;hypothetical 			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_13_3661_s_264	10850980	(iv) Most significantly, L-leucine specifically protects the archaeal Sa-Lrp binding capacity against irreversible heat inactivation; this effect likely reflects a physiologically significant interaction of leucine with the Sa-Lrp protein and suggests that leucine might function as the main effector of a hypothetical regulon.	bind
18415	1	5753	6	NULL	NULL	0	NULL	GSK-3beta	NULL		bind	NULL				AKAP220	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_40_36955_s_237	12147701	(iv) PP1 did not inhibit the binding of GSK-3beta to AKAP220.	bind
18416	2	5753	6	NULL	NULL	0	NULL	PP1	NULL		does not inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_40_36955_s_237	12147701	(iv) PP1 did not inhibit the binding of GSK-3beta to AKAP220.	bind
17548	1	5753	7	NULL	NULL	NULL	NULL	GSK-3beta	GP		binds to					AKAP220	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_40_36955_s_237	12147701	(iv) PP1 did not inhibit the binding of GSK-3beta to AKAP220.	bind
17549	2	5753	7	NULL	NULL	NULL	NULL	PP1	GP		does not inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_40_36955_s_237	12147701	(iv) PP1 did not inhibit the binding of GSK-3beta to AKAP220.	bind
18417	1	5754	6	10	NULL	0	NULL	TFIID protein	NULL	purified;;Yeast	bind	NULL					NULL			GATA sequence	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_23_17611_s_131	10748041	(iv) Purified yeast TFIID protein binds to a GATA sequence albeit less well than to a TATA sequence (Fig. 2 B of Ref.  27).	bind
18418	2	5754	6	10	NULL	0	NULL	TFIID protein	NULL	purified;;Yeast	bind	NULL					NULL			TATA sequence	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_23_17611_s_131	10748041	(iv) Purified yeast TFIID protein binds to a GATA sequence albeit less well than to a TATA sequence (Fig. 2 B of Ref.  27).	bind
18419	3	5754	6	NULL	NULL	0	NULL	statement 1	NULL		is less than	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_23_17611_s_131	10748041	(iv) Purified yeast TFIID protein binds to a GATA sequence albeit less well than to a TATA sequence (Fig. 2 B of Ref.  27).	bind
17550	1	5754	7	NULL	NULL	NULL	NULL	TFIID protein	GP	purified;;yeast	binds									GATA sequence	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_23_17611_s_131	10748041	(iv) Purified yeast TFIID protein binds to a GATA sequence albeit less well than to a TATA sequence (Fig. 2 B of Ref.  27).	bind
17551	2	5754	7	NULL	NULL	NULL	NULL	TFIID protein	GP	purified;;yeast	binds									TATA sequence	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_23_17611_s_131	10748041	(iv) Purified yeast TFIID protein binds to a GATA sequence albeit less well than to a TATA sequence (Fig. 2 B of Ref.  27).	bind
17552	3	5754	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs less well than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_23_17611_s_131	10748041	(iv) Purified yeast TFIID protein binds to a GATA sequence albeit less well than to a TATA sequence (Fig. 2 B of Ref.  27).	bind
18429	1	5755	6	NULL	NULL	0	NULL	SmF	NULL		bind	NULL				SmG	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_4_1956_s_246	9528767	(iv) SmE mutants unaffected in SmF and SmG binding (class IV).	bind
18430	2	5755	6	NULL	NULL	0	NULL	statement 1	NULL		has no effect on	NULL				SmE	NULL	mutant			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_4_1956_s_246	9528767	(iv) SmE mutants unaffected in SmF and SmG binding (class IV).	bind
17553	1	5755	7	NULL	NULL	NULL	NULL	SmF	GP		bind					SmG	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_1956_s_246	9528767	(iv) SmE mutants unaffected in SmF and SmG binding (class IV).	bind
17554	2	5755	7	NULL	NULL	NULL	NULL	statement 1	Process		does not affect					SmE	GP	mutants			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_1956_s_246	9528767	(iv) SmE mutants unaffected in SmF and SmG binding (class IV).	bind
18431	1	5756	6	10	NULL	0	NULL	CD14	NULL	radiolabeled	bind	NULL				LPS	NULL				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_71_1_61_s_9	12496149	(iv) SP-C enhances the binding of radiolabeled CD14 to LPS-coated wells.	bind
18432	2	5756	6	NULL	NULL	0	NULL	SP-C	NULL		enhances	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_71_1_61_s_9	12496149	(iv) SP-C enhances the binding of radiolabeled CD14 to LPS-coated wells.	bind
17555	1	5756	7	NULL	NULL	NULL	NULL	CD14	Cell	radiolabeled	bind					LPS	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_71_1_61_s_9	12496149	(iv) SP-C enhances the binding of radiolabeled CD14 to LPS-coated wells.	bind
17556	2	5756	7	NULL	NULL	NULL	NULL	SP-C	GP		enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_71_1_61_s_9	12496149	(iv) SP-C enhances the binding of radiolabeled CD14 to LPS-coated wells.	bind
18433	1	5757	6	NULL	NULL	0	NULL	SR-A	NULL		bind	NULL	directly			bacteria	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_4_1953_s_162	10722588	(iv) SR-A binds bacteria directly.	bind
17557	1	5757	7	NULL	NULL	NULL	NULL	SR-A	GP		binds		directly			bacteria	Organism				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_4_1953_s_162	10722588	(iv) SR-A binds bacteria directly.	bind
18434	1	5758	6	NULL	NULL	0	NULL	HKa	NULL		bind	NULL				urokinase receptor	NULL				NULL	vascular cell surface	0	NULL	NULL	NULL	gw60_jbiolchem_277_36_32677_s_182	12082110	(iv) The binding of HKa to the urokinase receptor ( 66) on vascular cell surfaces may approximate kallikrein and prourokinase and thereby potentiate plasmin formation.	bind
18435	2	5758	6	10	NULL	0	NULL	statement 1	NULL		potentiate	NULL				plasmin	NULL	formation of			NULL	vascular cell surface	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_36_32677_s_182	12082110	(iv) The binding of HKa to the urokinase receptor ( 66) on vascular cell surfaces may approximate kallikrein and prourokinase and thereby potentiate plasmin formation.	bind
18436	3	5758	6	NULL	NULL	0	NULL	statement 1	NULL		approximate	NULL	may			kallikrein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_36_32677_s_182	12082110	(iv) The binding of HKa to the urokinase receptor ( 66) on vascular cell surfaces may approximate kallikrein and prourokinase and thereby potentiate plasmin formation.	bind
18437	4	5758	6	NULL	NULL	0	NULL	statement 1	NULL		approximate	NULL	may			prourokinase	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_36_32677_s_182	12082110	(iv) The binding of HKa to the urokinase receptor ( 66) on vascular cell surfaces may approximate kallikrein and prourokinase and thereby potentiate plasmin formation.	bind
17558	1	5758	7	NULL	NULL	NULL	NULL	HKa	GP		bind					urokinase receptor	GP				NULL	vascular cell surface	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_36_32677_s_182	12082110	(iv) The binding of HKa to the urokinase receptor ( 66) on vascular cell surfaces may approximate kallikrein and prourokinase and thereby potentiate plasmin formation.	bind
17559	2	5758	7	NULL	NULL	NULL	NULL	statement 1	Process		approximate					kallikrein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_36_32677_s_182	12082110	(iv) The binding of HKa to the urokinase receptor ( 66) on vascular cell surfaces may approximate kallikrein and prourokinase and thereby potentiate plasmin formation.	bind
17560	3	5758	7	NULL	NULL	NULL	NULL	statement 1	Process		approximate					prourokinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_36_32677_s_182	12082110	(iv) The binding of HKa to the urokinase receptor ( 66) on vascular cell surfaces may approximate kallikrein and prourokinase and thereby potentiate plasmin formation.	bind
17561	4	5758	7	NULL	NULL	NULL	NULL	statement 1	Process		potentiate					plasmin	GP	formation of			NULL	vascular cell surface	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_36_32677_s_182	12082110	(iv) The binding of HKa to the urokinase receptor ( 66) on vascular cell surfaces may approximate kallikrein and prourokinase and thereby potentiate plasmin formation.	bind
18438	1	5759	6	NULL	NULL	0	NULL	IgI-MBP	NULL		bind	NULL				heparin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_15_10125_s_244	9092558	(iv) The binding of IgI-MBP and IgII-MBP to heparin, and of IgI-MBP to IgII-MBP, indicates that these protein constructs were folded in an active conformation.	bind
18439	2	5759	6	NULL	NULL	0	NULL	IgII-MBP	NULL		bind	NULL				heparin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_15_10125_s_244	9092558	(iv) The binding of IgI-MBP and IgII-MBP to heparin, and of IgI-MBP to IgII-MBP, indicates that these protein constructs were folded in an active conformation.	bind
18440	3	5759	6	NULL	NULL	0	NULL	IgI-MBP	NULL		bind	NULL				IgII-MBP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_15_10125_s_244	9092558	(iv) The binding of IgI-MBP and IgII-MBP to heparin, and of IgI-MBP to IgII-MBP, indicates that these protein constructs were folded in an active conformation.	bind
24583	4	5759	6	NULL	NULL	0	NULL	statement 1	NULL		indicate	NULL				IgI-MBP	NULL	active conformation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_15_10125_s_244	9092558	(iv) The binding of IgI-MBP and IgII-MBP to heparin, and of IgI-MBP to IgII-MBP, indicates that these protein constructs were folded in an active conformation.	bind
24584	5	5759	6	NULL	NULL	0	NULL	statement 2	NULL		indicate	NULL				IgI-MBP	NULL	active conformation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_15_10125_s_244	9092558	(iv) The binding of IgI-MBP and IgII-MBP to heparin, and of IgI-MBP to IgII-MBP, indicates that these protein constructs were folded in an active conformation.	bind
17563	1	5759	7	NULL	NULL	NULL	NULL	IgI-MBP	GP		bind					heparin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_15_10125_s_244	9092558	(iv) The binding of IgI-MBP and IgII-MBP to heparin, and of IgI-MBP to IgII-MBP, indicates that these protein constructs were folded in an active conformation.	bind
17564	2	5759	7	NULL	NULL	NULL	NULL	IgII-MBP	GP		bind					heparin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_15_10125_s_244	9092558	(iv) The binding of IgI-MBP and IgII-MBP to heparin, and of IgI-MBP to IgII-MBP, indicates that these protein constructs were folded in an active conformation.	bind
17565	3	5759	7	NULL	NULL	NULL	NULL	IgI-MBP	GP		bind					IgII-MBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_15_10125_s_244	9092558	(iv) The binding of IgI-MBP and IgII-MBP to heparin, and of IgI-MBP to IgII-MBP, indicates that these protein constructs were folded in an active conformation.	bind
17566	4	5759	7	NULL	NULL	NULL	NULL	statement 1	Process		indicate					IgI-MBP	GP	active conformation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_15_10125_s_244	9092558	(iv) The binding of IgI-MBP and IgII-MBP to heparin, and of IgI-MBP to IgII-MBP, indicates that these protein constructs were folded in an active conformation.	bind
17567	5	5759	7	NULL	NULL	NULL	NULL	statement 2	Process		indicate					IgII-MBP	GP	active conformation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_15_10125_s_244	9092558	(iv) The binding of IgI-MBP and IgII-MBP to heparin, and of IgI-MBP to IgII-MBP, indicates that these protein constructs were folded in an active conformation.	bind
24580	1	5760	6	10	NULL	0	NULL	HMR-E silencer	NULL		is a type of	NULL			E element		NULL			Rap1 binding site	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_11_4514_s_375	15899856	(iv) The E element of the  HMR-E silencer is a binding site for Rap1 ( ), so if a defect in the binding of Rap1 to Sir4 was the cause of the phenotypes of the  sir4 coiled-coil mutants, than we would predict that the silencing defects of these mutants in a  hmrdeltaE strain would be no more severe than  hmrdeltaE in a  SIR4 strain.	bind
24581	2	5760	6	NULL	NULL	0	NULL	Rap1	NULL		bind	NULL				Sir4	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_11_4514_s_375	15899856	(iv) The E element of the  HMR-E silencer is a binding site for Rap1 ( ), so if a defect in the binding of Rap1 to Sir4 was the cause of the phenotypes of the  sir4 coiled-coil mutants, than we would predict that the silencing defects of these mutants in a  hmrdeltaE strain would be no more severe than  hmrdeltaE in a  SIR4 strain.	bind
24582	3	5760	6	NULL	NULL	0	NULL	statement 2	NULL	defect in	cause	NULL				sir4 phenotypes	NULL	coiled coil mutant			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_11_4514_s_375	15899856	(iv) The E element of the  HMR-E silencer is a binding site for Rap1 ( ), so if a defect in the binding of Rap1 to Sir4 was the cause of the phenotypes of the  sir4 coiled-coil mutants, than we would predict that the silencing defects of these mutants in a  hmrdeltaE strain would be no more severe than  hmrdeltaE in a  SIR4 strain.	bind
17568	1	5760	7	NULL	NULL	NULL	NULL	HMR-E silencer	GP		is a type of				 E element  					Rap1binding site	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_11_4514_s_375	15899856	(iv) The E element of the  HMR-E silencer is a binding site for Rap1 ( ), so if a defect in the binding of Rap1 to Sir4 was the cause of the phenotypes of the  sir4 coiled-coil mutants, than we would predict that the silencing defects of these mutants in a  hmrdeltaE strain would be no more severe than  hmrdeltaE in a  SIR4 strain.	bind
17569	2	5760	7	NULL	NULL	NULL	NULL	Rap1	GP		bind					Sir4	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_11_4514_s_375	15899856	(iv) The E element of the  HMR-E silencer is a binding site for Rap1 ( ), so if a defect in the binding of Rap1 to Sir4 was the cause of the phenotypes of the  sir4 coiled-coil mutants, than we would predict that the silencing defects of these mutants in a  hmrdeltaE strain would be no more severe than  hmrdeltaE in a  SIR4 strain.	bind
17656	3	5760	7	NULL	NULL	NULL	NULL	statement 2	Process	defect in	cause					sir4 phenotypes	Process	coiled-coil mutant 			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_11_4514_s_375	15899856	(iv) The E element of the  HMR-E silencer is a binding site for Rap1 ( ), so if a defect in the binding of Rap1 to Sir4 was the cause of the phenotypes of the  sir4 coiled-coil mutants, than we would predict that the silencing defects of these mutants in a  hmrdeltaE strain would be no more severe than  hmrdeltaE in a  SIR4 strain.	bind
18442	1	5762	6	NULL	NULL	0	NULL	tRNA	NULL	uncharged 	bind	NULL				Gcn2	NULL		HisRS domain		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_12_8422_s_355	10567567	(iv) Upon amino acid starvation, uncharged tRNA binds to the HisRS domain of Gcn2 and induces a conformational change that results in the release of Hsp90.	bind
18443	2	5762	6	10	NULL	0	NULL	statement 1	NULL		occurs upon	NULL				amino acid 	NULL	starvation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8422_s_355	10567567	(iv) Upon amino acid starvation, uncharged tRNA binds to the HisRS domain of Gcn2 and induces a conformational change that results in the release of Hsp90.	bind
18444	3	5762	6	10	NULL	0	NULL	statement 1	NULL		induces a 	NULL				conformational change	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8422_s_355	10567567	(iv) Upon amino acid starvation, uncharged tRNA binds to the HisRS domain of Gcn2 and induces a conformational change that results in the release of Hsp90.	bind
45760	4	5762	6	10	NULL	0	NULL	statement 3	NULL		results in	NULL				Hsp90	NULL	release of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_12_8422_s_355	10567567	(iv) Upon amino acid starvation, uncharged tRNA binds to the HisRS domain of Gcn2 and induces a conformational change that results in the release of Hsp90.	bind
17575	1	5762	7	NULL	NULL	NULL	NULL	tRNA	NucleicAcid	uncharged	binds to					Gcn2	GP		HisRS domain		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8422_s_355	10567567	(iv) Upon amino acid starvation, uncharged tRNA binds to the HisRS domain of Gcn2 and induces a conformational change that results in the release of Hsp90.	bind
17576	2	5762	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs upon					aminoacid	AminoAcid	starvation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8422_s_355	10567567	(iv) Upon amino acid starvation, uncharged tRNA binds to the HisRS domain of Gcn2 and induces a conformational change that results in the release of Hsp90.	bind
17577	4	5762	7	NULL	NULL	NULL	NULL	statement 3	Process		results in					Hsp90	GP	release of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8422_s_355	10567567	(iv) Upon amino acid starvation, uncharged tRNA binds to the HisRS domain of Gcn2 and induces a conformational change that results in the release of Hsp90.	bind
17578	3	5762	7	NULL	NULL	NULL	NULL	statement 1	Process		induce					conformational change 	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8422_s_355	10567567	(iv) Upon amino acid starvation, uncharged tRNA binds to the HisRS domain of Gcn2 and induces a conformational change that results in the release of Hsp90.	bind
18445	1	5763	6	NULL	NULL	0	NULL	heparin	NULL		bind	NULL				VN	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_53_37611_s_30	10608816	(iv) what are the kinetics parameters of heparin binding to VN?	bind
17582	1	5763	7	NULL	NULL	NULL	NULL	heparin 	GP		bind					VN	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_53_37611_s_30	10608816	(iv) what are the kinetics parameters of heparin binding to VN?	bind
18446	1	5764	6	NULL	NULL	0	NULL	BHK cells	NULL	transfected	overexpress	NULL				LRP	NULL				NULL	cell surface	0	NULL	NULL	NULL	gw60_embo_20_21_5863_s_186	11689427	(J - M) Increased PrP-binding by rec. SFV RNA transfected BHK cells overexpressing LRP at the cell surface.	bind
18447	2	5764	6	10	NULL	0	NULL	rec. SFV RNA	NULL		increased	NULL				PrP	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_21_5863_s_186	11689427	(J - M) Increased PrP-binding by rec. SFV RNA transfected BHK cells overexpressing LRP at the cell surface.	bind
17583	1	5764	7	NULL	NULL	NULL	NULL	BHK cells	Cell		is transfected with					SFV RNA	NucleicAcid	rec			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_21_5863_s_186	11689427	(J - M) Increased PrP-binding by rec. SFV RNA transfected BHK cells overexpressing LRP at the cell surface.	bind
17584	2	5764	7	NULL	NULL	NULL	NULL	statement 1	Process		overexpress					LRP	GP				NULL	cell surface	NULL	NULL	NULL	NULL	gw60_embo_20_21_5863_s_186	11689427	(J - M) Increased PrP-binding by rec. SFV RNA transfected BHK cells overexpressing LRP at the cell surface.	bind
45856	3	5764	7	NULL	NULL	NULL	NULL	statement 2	Process		increases					Prp	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_21_5863_s_186	11689427	(J - M) Increased PrP-binding by rec. SFV RNA transfected BHK cells overexpressing LRP at the cell surface.	bind
18448	1	5765	6	NULL	NULL	0	NULL	Isl1	NULL		bind	NULL					NULL			MNE	NULL		0	NULL	NULL	NULL	gw60_neuron_38_5_731_s_199	12797958	(J) The binding of Isl1 and Lhx3 to MNE was analyzed by chromatin immune precipitation analysis.	bind
18449	2	5765	6	NULL	NULL	0	NULL	Lhx3	NULL		bind	NULL					NULL			MNE	NULL		0	NULL	NULL	NULL	gw60_neuron_38_5_731_s_199	12797958	(J) The binding of Isl1 and Lhx3 to MNE was analyzed by chromatin immune precipitation analysis.	bind
17585	1	5765	7	NULL	NULL	NULL	NULL	Isl1	GP		bind									MNE	NULL		NULL	NULL	NULL	NULL	gw60_neuron_38_5_731_s_199	12797958	(J) The binding of Isl1 and Lhx3 to MNE was analyzed by chromatin immune precipitation analysis.	bind
17586	2	5765	7	NULL	NULL	NULL	NULL	Lhx3	GP		bind									MNE	NULL		NULL	NULL	NULL	NULL	gw60_neuron_38_5_731_s_199	12797958	(J) The binding of Isl1 and Lhx3 to MNE was analyzed by chromatin immune precipitation analysis.	bind
18450	1	5766	6	10	NULL	0	NULL	Spo0J-GFP			bind					PSL23 strain				parS	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_4_1326_s_168	12562803	(J, K) Position of Spo0J-GFP bound to a  parS array (J, strain PSL23) or LacI-CFP bound to a  lac operator array (K, strain KPL716) inserted at 270 degrees .	bind
18451	2	5766	6	10	NULL	0	NULL	LacI-CFP			bind					KPL716 strain				lac operator	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_4_1326_s_168	12562803	(J, K) Position of Spo0J-GFP bound to a  parS array (J, strain PSL23) or LacI-CFP bound to a  lac operator array (K, strain KPL716) inserted at 270 degrees .	bind
17589	1	5766	7	NULL	NULL	NULL	NULL	Spo0J-GFP	GP		bind					PSL23	GP			parS 	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_4_1326_s_168	12562803	(J, K) Position of Spo0J-GFP bound to a  parS array (J, strain PSL23) or LacI-CFP bound to a  lac operator array (K, strain KPL716) inserted at 270 degrees .	bind
17591	2	5766	7	NULL	NULL	NULL	NULL	LacI-CFP	GP		bind					strain KPL716	Organism			lac operator	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_4_1326_s_168	12562803	(J, K) Position of Spo0J-GFP bound to a  parS array (J, strain PSL23) or LacI-CFP bound to a  lac operator array (K, strain KPL716) inserted at 270 degrees .	bind
18452	1	5767	6	NULL	NULL	0	NULL	HOXA13	NULL	wild type	bind	NULL				Bmp2	NULL			enhancer	NULL	developing limbs	NULL	NULL	NULL	NULL	gw70_development_131_18_4581_s_154	15342482	(J-L) Chromatin immunoprecipitation  using the  Hoxa13 antibody confirms that wild-type (+/+) HOXA13 binds the  Bmp2 (J) and  Bmp7s1 (K) enhancer regions in the developing limb, whereas immunoprecipitates from mutant  limbs ( - / - ) lacking the HOXA13 DNA-binding domain did not contain the  Bmp2 and  Bmp7s1 enhancer regions.	bind
18453	2	5767	6	NULL	NULL	0	NULL	HOXA13	NULL	wild type	bind	NULL				Bmp7s1	NULL			enhancer	NULL	developing limbs	NULL	NULL	NULL	NULL	gw70_development_131_18_4581_s_154	15342482	(J-L) Chromatin immunoprecipitation  using the  Hoxa13 antibody confirms that wild-type (+/+) HOXA13 binds the  Bmp2 (J) and  Bmp7s1 (K) enhancer regions in the developing limb, whereas immunoprecipitates from mutant  limbs ( - / - ) lacking the HOXA13 DNA-binding domain did not contain the  Bmp2 and  Bmp7s1 enhancer regions.	bind
18454	3	5767	6	NULL	NULL	0	NULL	HOXA13	NULL	mutant	does not bind	NULL				Bmp2 	NULL			enhancer	NULL	developing limbs	NULL	NULL	NULL	NULL	gw70_development_131_18_4581_s_154	15342482	(J-L) Chromatin immunoprecipitation  using the  Hoxa13 antibody confirms that wild-type (+/+) HOXA13 binds the  Bmp2 (J) and  Bmp7s1 (K) enhancer regions in the developing limb, whereas immunoprecipitates from mutant  limbs ( - / - ) lacking the HOXA13 DNA-binding domain did not contain the  Bmp2 and  Bmp7s1 enhancer regions.	bind
18455	4	5767	6	NULL	NULL	0	NULL	HOXA13	NULL	mutant	does not bind	NULL				Bmp7s1	NULL			enhancer	NULL	developing limbs	NULL	NULL	NULL	NULL	gw70_development_131_18_4581_s_154	15342482	(J-L) Chromatin immunoprecipitation  using the  Hoxa13 antibody confirms that wild-type (+/+) HOXA13 binds the  Bmp2 (J) and  Bmp7s1 (K) enhancer regions in the developing limb, whereas immunoprecipitates from mutant  limbs ( - / - ) lacking the HOXA13 DNA-binding domain did not contain the  Bmp2 and  Bmp7s1 enhancer regions.	bind
53248	5	5767	6	10	NULL	0	NULL	HOXA13	NULL	mutant	lacks	NULL					NULL		DNA-binding domain		NULL		0	NULL	NULL	NULL	gw70_development_131_18_4581_s_154	15342482	(J-L) Chromatin immunoprecipitation  using the  Hoxa13 antibody confirms that wild-type (+/+) HOXA13 binds the  Bmp2 (J) and  Bmp7s1 (K) enhancer regions in the developing limb, whereas immunoprecipitates from mutant  limbs ( - / - ) lacking the HOXA13 DNA-binding domain did not contain the  Bmp2 and  Bmp7s1 enhancer regions.	bind
17594	1	5767	7	NULL	NULL	NULL	NULL	HOXA13	GP	wild-type	binds					Bmp2 	GP			enhancer	NULL	in the developing limb	NULL	NULL	NULL	NULL	gw70_development_131_18_4581_s_154	15342482	(J-L) Chromatin immunoprecipitation  using the  Hoxa13 antibody confirms that wild-type (+/+) HOXA13 binds the  Bmp2 (J) and  Bmp7s1 (K) enhancer regions in the developing limb, whereas immunoprecipitates from mutant  limbs ( - / - ) lacking the HOXA13 DNA-binding domain did not contain the  Bmp2 and  Bmp7s1 enhancer regions.	bind
17595	2	5767	7	NULL	NULL	NULL	NULL	HOXA13	GP	wild-type	binds					Bmp7s1	GP			enhancer	NULL	in the developing limb	NULL	NULL	NULL	NULL	gw70_development_131_18_4581_s_154	15342482	(J-L) Chromatin immunoprecipitation  using the  Hoxa13 antibody confirms that wild-type (+/+) HOXA13 binds the  Bmp2 (J) and  Bmp7s1 (K) enhancer regions in the developing limb, whereas immunoprecipitates from mutant  limbs ( - / - ) lacking the HOXA13 DNA-binding domain did not contain the  Bmp2 and  Bmp7s1 enhancer regions.	bind
17596	3	5767	7	NULL	NULL	NULL	NULL	HOXA13	GP	mutant	does not bind					Bmp2	GP			enhancer	NULL	developing limb	NULL	NULL	NULL	NULL	gw70_development_131_18_4581_s_154	15342482	(J-L) Chromatin immunoprecipitation  using the  Hoxa13 antibody confirms that wild-type (+/+) HOXA13 binds the  Bmp2 (J) and  Bmp7s1 (K) enhancer regions in the developing limb, whereas immunoprecipitates from mutant  limbs ( - / - ) lacking the HOXA13 DNA-binding domain did not contain the  Bmp2 and  Bmp7s1 enhancer regions.	bind
17597	4	5767	7	NULL	NULL	NULL	NULL	HOXA13	GP	mutant	does not bind					Bmp7s1	GP			enhancer	NULL	developing limb	NULL	NULL	NULL	NULL	gw70_development_131_18_4581_s_154	15342482	(J-L) Chromatin immunoprecipitation  using the  Hoxa13 antibody confirms that wild-type (+/+) HOXA13 binds the  Bmp2 (J) and  Bmp7s1 (K) enhancer regions in the developing limb, whereas immunoprecipitates from mutant  limbs ( - / - ) lacking the HOXA13 DNA-binding domain did not contain the  Bmp2 and  Bmp7s1 enhancer regions.	bind
53247	5	5767	7	NULL	NULL	NULL	NULL	HOXA13	GP	mutant	lacks								DNA-binding domain		NULL		NULL	NULL	NULL	NULL	gw70_development_131_18_4581_s_154	15342482	(J-L) Chromatin immunoprecipitation  using the  Hoxa13 antibody confirms that wild-type (+/+) HOXA13 binds the  Bmp2 (J) and  Bmp7s1 (K) enhancer regions in the developing limb, whereas immunoprecipitates from mutant  limbs ( - / - ) lacking the HOXA13 DNA-binding domain did not contain the  Bmp2 and  Bmp7s1 enhancer regions.	bind
18456	1	5768	6	10	NULL	0	NULL	DC3B ADP	NULL	prolonged treatment of	ribosylates	NULL				RhoA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_8_12_2437_s_164	9398666	(Just  et al., 1993  ; Gong  et al., 1996  ; present study), and our finding that prolonged treatment of DC3B ADP-ribosylates RhoA that reassociates with rhoGDI is consistent with a previous study that showed that RhoA ADP ribosylated in vitro can bind to rhoGDI (Hancock and Hall, 1993  ).	bind
18457	2	5768	6	NULL	NULL	0	NULL	RhoA	NULL		reassociates with	NULL				rhoGDI	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_8_12_2437_s_164	9398666	(Just  et al., 1993  ; Gong  et al., 1996  ; present study), and our finding that prolonged treatment of DC3B ADP-ribosylates RhoA that reassociates with rhoGDI is consistent with a previous study that showed that RhoA ADP ribosylated in vitro can bind to rhoGDI (Hancock and Hall, 1993  ).	bind
18458	3	5768	6	NULL	NULL	0	NULL	RhoA ADP	NULL	ribosylated	bind	NULL				rhoGDI	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_molbiolcell_8_12_2437_s_164	9398666	(Just  et al., 1993  ; Gong  et al., 1996  ; present study), and our finding that prolonged treatment of DC3B ADP-ribosylates RhoA that reassociates with rhoGDI is consistent with a previous study that showed that RhoA ADP ribosylated in vitro can bind to rhoGDI (Hancock and Hall, 1993  ).	bind
17598	1	5768	7	NULL	NULL	NULL	NULL	DC3B ADP	GP	prolonged treatment of	ribosylates					RhoA	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_8_12_2437_s_164	9398666	(Just  et al., 1993  ; Gong  et al., 1996  ; present study), and our finding that prolonged treatment of DC3B ADP-ribosylates RhoA that reassociates with rhoGDI is consistent with a previous study that showed that RhoA ADP ribosylated in vitro can bind to rhoGDI (Hancock and Hall, 1993  ).	bind
17599	2	5768	7	NULL	NULL	NULL	NULL	statement 1	Process		reassociate with					rhoGDI	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_8_12_2437_s_164	9398666	(Just  et al., 1993  ; Gong  et al., 1996  ; present study), and our finding that prolonged treatment of DC3B ADP-ribosylates RhoA that reassociates with rhoGDI is consistent with a previous study that showed that RhoA ADP ribosylated in vitro can bind to rhoGDI (Hancock and Hall, 1993  ).	bind
17600	3	5768	7	NULL	NULL	NULL	NULL	RhoA ADP 	GP	ribosylated	bind					rhoGDI	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molbiolcell_8_12_2437_s_164	9398666	(Just  et al., 1993  ; Gong  et al., 1996  ; present study), and our finding that prolonged treatment of DC3B ADP-ribosylates RhoA that reassociates with rhoGDI is consistent with a previous study that showed that RhoA ADP ribosylated in vitro can bind to rhoGDI (Hancock and Hall, 1993  ).	bind
18459	1	5769	6	NULL	NULL	0	NULL	m-UBR2	NULL		bind	NULL				HR6B E2 enzyme	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_22_8255_s_40	14585983	(K) m-UBR2 binds to the HR6B E2  enzyme.	bind
17603	1	5769	7	NULL	NULL	NULL	NULL	m-UBR2	GP		binds to					HR6B E2 enzyme	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_22_8255_s_40	14585983	(K) m-UBR2 binds to the HR6B E2  enzyme.	bind
18460	1	5770	6	NULL	NULL	0	NULL	Su(H)	NULL		bind	NULL					NULL			SME	NULL		0	NULL	NULL	NULL	gw60_cell_103_1_75_s_218	11051549	(K) Su(H) binding to the  SME.	bind
17606	1	5770	7	NULL	NULL	NULL	NULL	Su(H)	GP		bind									SME	NULL		NULL	NULL	NULL	NULL	gw60_cell_103_1_75_s_218	11051549	(K) Su(H) binding to the  SME.	bind
18461	1	5771	6	NULL	NULL	0	NULL	Dll3	NULL		localizes	NULL				Mesp2	NULL	expression of			NULL		0	NULL	NULL	NULL	gw60_development_130_18_4259_s_176	12900443	(K,L) Dll3 is required for localization of  Mesp2 expression into the rostral half of somites.	bind
18462	2	5771	6	NULL	NULL	0	NULL	Mesp2	NULL		expressed into	NULL				rostral half of somites	NULL				NULL		0	NULL	NULL	NULL	gw60_development_130_18_4259_s_176	12900443	(K,L) Dll3 is required for localization of  Mesp2 expression into the rostral half of somites.	bind
17607	1	5771	7	NULL	NULL	NULL	NULL	Dll3	GP		localizes					Mesp2	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_development_130_18_4259_s_176	12900443	(K,L) Dll3 is required for localization of  Mesp2 expression into the rostral half of somites.	bind
25023	2	5771	7	NULL	NULL	NULL	NULL	Mesp2	GP		expressed into					rostral half of somites	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_development_130_18_4259_s_176	12900443	(K,L) Dll3 is required for localization of  Mesp2 expression into the rostral half of somites.	bind
18472	1	5773	6	NULL	NULL	0	NULL	Kelch-like ECH-associated protein 1	NULL		bind	NULL				Nrf2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_27244_s_26	15917255	(Kelch-like ECH-associated protein 1) binds to Nrf2 and facilitates the degradation of Nrf2 via the proteasome system ( ).	bind
18473	2	5773	6	10	NULL	0	NULL	statement 1	NULL		facilitate	NULL				Nrf2	NULL	degradation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_29_27244_s_26	15917255	(Kelch-like ECH-associated protein 1) binds to Nrf2 and facilitates the degradation of Nrf2 via the proteasome system ( ).	bind
18474	3	5773	6	NULL	NULL	0	NULL	statement 2	NULL		occurs via 	NULL				proteasome system	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_27244_s_26	15917255	(Kelch-like ECH-associated protein 1) binds to Nrf2 and facilitates the degradation of Nrf2 via the proteasome system ( ).	bind
17611	1	5773	7	NULL	NULL	NULL	NULL	Kelch-like ECH-associated protein 1	GP		binds to					Nrf2 	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_29_27244_s_26	15917255	(Kelch-like ECH-associated protein 1) binds to Nrf2 and facilitates the degradation of Nrf2 via the proteasome system ( ).	bind
17612	2	5773	7	NULL	NULL	NULL	NULL	statement 1	Process		facilitate					Nrf2 	GP	degradation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_29_27244_s_26	15917255	(Kelch-like ECH-associated protein 1) binds to Nrf2 and facilitates the degradation of Nrf2 via the proteasome system ( ).	bind
17613	3	5773	7	NULL	NULL	NULL	NULL	statement 2	Process		occurs via					proteasome system	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_29_27244_s_26	15917255	(Kelch-like ECH-associated protein 1) binds to Nrf2 and facilitates the degradation of Nrf2 via the proteasome system ( ).	bind
18476	1	5774	6	10	NULL	0	NULL	telomerase RNA variant	NULL	deletion 	bind	NULL		stem loop IV		TERT	NULL				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_13_9_1116_s_71	10323863	(Lane  1) No competitor; (lane  2) a telomerase RNA variant missing stem-loop IV, which binds TERT but is less active than the wild-type RNA (see Results); (lanes  3,4) tRNA; (lanes  5,6) 5S RNA; (lanes  7,8) total yeast RNA; (lanes  9,10) a 24-nucleotide RNA oligonucleotide representing telomerase RNA residues 36-59 which have no activity (Collins and Gandhi 1998  ).	bind
45761	2	5774	6	10	NULL	0	NULL	statement 1	NULL		is less active than	NULL				RNA	NULL	wild type			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_13_9_1116_s_71	10323863	(Lane  1) No competitor; (lane  2) a telomerase RNA variant missing stem-loop IV, which binds TERT but is less active than the wild-type RNA (see Results); (lanes  3,4) tRNA; (lanes  5,6) 5S RNA; (lanes  7,8) total yeast RNA; (lanes  9,10) a 24-nucleotide RNA oligonucleotide representing telomerase RNA residues 36-59 which have no activity (Collins and Gandhi 1998  ).	bind
17614	1	5774	7	NULL	NULL	NULL	NULL	telomerase RNA variant	NucleicAcid		missing					stem-loop IV	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_13_9_1116_s_71	10323863	(Lane  1) No competitor; (lane  2) a telomerase RNA variant missing stem-loop IV, which binds TERT but is less active than the wild-type RNA (see Results); (lanes  3,4) tRNA; (lanes  5,6) 5S RNA; (lanes  7,8) total yeast RNA; (lanes  9,10) a 24-nucleotide RNA oligonucleotide representing telomerase RNA residues 36-59 which have no activity (Collins and Gandhi 1998  ).	bind
17615	2	5774	7	NULL	NULL	NULL	NULL	statement 1	Process		binds					TERT	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_13_9_1116_s_71	10323863	(Lane  1) No competitor; (lane  2) a telomerase RNA variant missing stem-loop IV, which binds TERT but is less active than the wild-type RNA (see Results); (lanes  3,4) tRNA; (lanes  5,6) 5S RNA; (lanes  7,8) total yeast RNA; (lanes  9,10) a 24-nucleotide RNA oligonucleotide representing telomerase RNA residues 36-59 which have no activity (Collins and Gandhi 1998  ).	bind
17617	3	5774	7	NULL	NULL	NULL	NULL	statement 2	Process		is less active than					RNA	NucleicAcid	wild-type			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_13_9_1116_s_71	10323863	(Lane  1) No competitor; (lane  2) a telomerase RNA variant missing stem-loop IV, which binds TERT but is less active than the wild-type RNA (see Results); (lanes  3,4) tRNA; (lanes  5,6) 5S RNA; (lanes  7,8) total yeast RNA; (lanes  9,10) a 24-nucleotide RNA oligonucleotide representing telomerase RNA residues 36-59 which have no activity (Collins and Gandhi 1998  ).	bind
18477	1	5775	6	10	NULL	0	NULL	Pse1-GFP	NULL		bind	NULL				Pho4	NULL	WT			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_17_2673_s_126	9732266	(Lane  1) Three percent of the Pse1-GFP extract loaded (L); (lane  2) Pse1-GFP bound to Pho4WT-zz (WT); (lane  3) Pse1-GFP bound to Pho4delta157-164-zz (delta); (lane  4) Pse1-GFP bound to IgG-Sepharose beads ( ).	bind
18478	2	5775	6	NULL	NULL	0	NULL	Pse1-GFP	NULL		bind	NULL				Pho4	NULL		delta157-164		NULL		0	NULL	NULL	NULL	gw60_genesdev_12_17_2673_s_126	9732266	(Lane  1) Three percent of the Pse1-GFP extract loaded (L); (lane  2) Pse1-GFP bound to Pho4WT-zz (WT); (lane  3) Pse1-GFP bound to Pho4delta157-164-zz (delta); (lane  4) Pse1-GFP bound to IgG-Sepharose beads ( ).	bind
17618	1	5775	7	NULL	NULL	NULL	NULL	Pse1-GFP	GP		bind					Pho4	GP	WT	zz		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_17_2673_s_126	9732266	(Lane  1) Three percent of the Pse1-GFP extract loaded (L); (lane  2) Pse1-GFP bound to Pho4WT-zz (WT); (lane  3) Pse1-GFP bound to Pho4delta157-164-zz (delta); (lane  4) Pse1-GFP bound to IgG-Sepharose beads ( ).	bind
17619	2	5775	7	NULL	NULL	NULL	NULL	Pse1-GFP	GP		bind					Pho4	GP		delta 157-164-zz 		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_17_2673_s_126	9732266	(Lane  1) Three percent of the Pse1-GFP extract loaded (L); (lane  2) Pse1-GFP bound to Pho4WT-zz (WT); (lane  3) Pse1-GFP bound to Pho4delta157-164-zz (delta); (lane  4) Pse1-GFP bound to IgG-Sepharose beads ( ).	bind
18479	1	5776	6	NULL	NULL	0	NULL	Oct4	NULL		bind	NULL				UTF1	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_17_16_2048_s_37	12923055	(Lanes   3 -  7)  Increasing amounts of Sox2-HMG protein mixed with equal amounts of Oct4 + DNA.   Although Oct4 binds alone to  UTF1 significantly more weakly than to   FGF4 (cf. the two lane  2s), heterodimerization on   UTF1 is more pronounced with even lower amounts of Sox2 (e.g., cf.  the two lane  4s or  5s).	bind
18480	2	5776	6	NULL	NULL	0	NULL	Oct4	NULL		bind	NULL				FGF4	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_17_16_2048_s_37	12923055	(Lanes   3 -  7)  Increasing amounts of Sox2-HMG protein mixed with equal amounts of Oct4 + DNA.   Although Oct4 binds alone to  UTF1 significantly more weakly than to   FGF4 (cf. the two lane  2s), heterodimerization on   UTF1 is more pronounced with even lower amounts of Sox2 (e.g., cf.  the two lane  4s or  5s).	bind
18481	3	5776	6	NULL	NULL	0	NULL	statement 1	NULL		is more weak than	NULL	significantly			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_17_16_2048_s_37	12923055	(Lanes   3 -  7)  Increasing amounts of Sox2-HMG protein mixed with equal amounts of Oct4 + DNA.   Although Oct4 binds alone to  UTF1 significantly more weakly than to   FGF4 (cf. the two lane  2s), heterodimerization on   UTF1 is more pronounced with even lower amounts of Sox2 (e.g., cf.  the two lane  4s or  5s).	bind
17621	1	5776	7	NULL	NULL	NULL	NULL	Oct4	GP		binds to					UTF1 	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_16_2048_s_37	12923055	(Lanes   3 -  7)  Increasing amounts of Sox2-HMG protein mixed with equal amounts of Oct4 + DNA.   Although Oct4 binds alone to  UTF1 significantly more weakly than to   FGF4 (cf. the two lane  2s), heterodimerization on   UTF1 is more pronounced with even lower amounts of Sox2 (e.g., cf.  the two lane  4s or  5s).	bind
17622	2	5776	7	NULL	NULL	NULL	NULL	Oct4	GP		binds to					FGF4	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_16_2048_s_37	12923055	(Lanes   3 -  7)  Increasing amounts of Sox2-HMG protein mixed with equal amounts of Oct4 + DNA.   Although Oct4 binds alone to  UTF1 significantly more weakly than to   FGF4 (cf. the two lane  2s), heterodimerization on   UTF1 is more pronounced with even lower amounts of Sox2 (e.g., cf.  the two lane  4s or  5s).	bind
17623	3	5776	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs  more weakly than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_16_2048_s_37	12923055	(Lanes   3 -  7)  Increasing amounts of Sox2-HMG protein mixed with equal amounts of Oct4 + DNA.   Although Oct4 binds alone to  UTF1 significantly more weakly than to   FGF4 (cf. the two lane  2s), heterodimerization on   UTF1 is more pronounced with even lower amounts of Sox2 (e.g., cf.  the two lane  4s or  5s).	bind
17624	4	5776	7	NULL	NULL	NULL	NULL	UTF1	GP	heterodimerization on	occurs with					Sox2	GP	even lower amounts of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_16_2048_s_37	12923055	(Lanes   3 -  7)  Increasing amounts of Sox2-HMG protein mixed with equal amounts of Oct4 + DNA.   Although Oct4 binds alone to  UTF1 significantly more weakly than to   FGF4 (cf. the two lane  2s), heterodimerization on   UTF1 is more pronounced with even lower amounts of Sox2 (e.g., cf.  the two lane  4s or  5s).	bind
18482	1	5777	6	NULL	NULL	0	NULL	Lhx3	NULL		bind	NULL				Isl1	NULL		C-terminal		NULL		0	NULL	NULL	NULL	gw60_cell_110_2_237_s_213	12150931	(Lanes 3 and 4) NLI is a competitor for Lhx3 binding to C-terminal Isl1.	bind
18483	2	5777	6	NULL	NULL	0	NULL	NLI	NULL		bind	NULL				Isl1	NULL		C-terminal		NULL		0	NULL	NULL	NULL	gw60_cell_110_2_237_s_213	12150931	(Lanes 3 and 4) NLI is a competitor for Lhx3 binding to C-terminal Isl1.	bind
18484	3	5777	6	NULL	NULL	0	NULL	statement 1	NULL		competes	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_110_2_237_s_213	12150931	(Lanes 3 and 4) NLI is a competitor for Lhx3 binding to C-terminal Isl1.	bind
17626	1	5777	7	NULL	NULL	NULL	NULL	Lhx3	GP		bind					Isl1	GP		C-terminal		NULL		NULL	NULL	NULL	NULL	gw60_cell_110_2_237_s_213	12150931	(Lanes 3 and 4) NLI is a competitor for Lhx3 binding to C-terminal Isl1.	bind
17627	2	5777	7	NULL	NULL	NULL	NULL	NLI	GP		bind					Isl1	GP		C-terminal		NULL		NULL	NULL	NULL	NULL	gw60_cell_110_2_237_s_213	12150931	(Lanes 3 and 4) NLI is a competitor for Lhx3 binding to C-terminal Isl1.	bind
45857	3	5777	7	NULL	NULL	NULL	NULL	statement 2	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_110_2_237_s_213	12150931	(Lanes 3 and 4) NLI is a competitor for Lhx3 binding to C-terminal Isl1.	bind
18485	1	5778	6	NULL	NULL	0	NULL	p16	NULL		bind	NULL				cdk4	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3916_s_215	10207115	(Left panel) Binding of p16 to cdk4.	bind
17628	1	5778	7	NULL	NULL	NULL	NULL	p16	GP		bind					cdk4	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3916_s_215	10207115	(Left panel) Binding of p16 to cdk4.	bind
18486	1	5779	6	10	NULL	0	NULL		NULL		bind	NULL		CFP-PH 		PIP2	NULL				NULL	resting cell membrane	NULL	NULL	NULL	NULL	gw70_embo_24_9_1664_s_46	15861130	(Left panel) In a resting cell, CFP-PH and YFP-PH bind to PIP2 at the membrane and FRET occurs.	bind
18487	2	5779	6	10	NULL	0	NULL		NULL		bind	NULL		YFP-PH		PIP2	NULL				NULL	resting cell membrane	NULL	NULL	NULL	NULL	gw70_embo_24_9_1664_s_46	15861130	(Left panel) In a resting cell, CFP-PH and YFP-PH bind to PIP2 at the membrane and FRET occurs.	bind
17629	1	5779	7	NULL	NULL	NULL	NULL				bind			CFP-PH		PIP2	Chemical				NULL	resting cell membrane	NULL	NULL	NULL	NULL	gw70_embo_24_9_1664_s_46	15861130	(Left panel) In a resting cell, CFP-PH and YFP-PH bind to PIP2 at the membrane and FRET occurs.	bind
17630	2	5779	7	NULL	NULL	NULL	NULL				bind			YFP-PH		PIP2	Chemical				NULL	resting cell membrane	NULL	NULL	NULL	NULL	gw70_embo_24_9_1664_s_46	15861130	(Left panel) In a resting cell, CFP-PH and YFP-PH bind to PIP2 at the membrane and FRET occurs.	bind
18488	1	5780	6	10	NULL	0	NULL	Nuc	NULL		bind	NULL		RGG		G4 DNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_11_2944_s_53	12771220	(Left) Distamycin inhibition of binding of Nuc-RGG to G4 DNA.	bind
18489	2	5780	6	NULL	NULL	0	NULL	Distamycin	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_11_2944_s_53	12771220	(Left) Distamycin inhibition of binding of Nuc-RGG to G4 DNA.	bind
17631	1	5780	7	NULL	NULL	NULL	NULL	Nuc	GP		bind			RGG		G4 DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_11_2944_s_53	12771220	(Left) Distamycin inhibition of binding of Nuc-RGG to G4 DNA.	bind
17632	2	5780	7	NULL	NULL	NULL	NULL	Distamycin	Chemical		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_11_2944_s_53	12771220	(Left) Distamycin inhibition of binding of Nuc-RGG to G4 DNA.	bind
18490	1	5781	6	10	NULL	0	NULL	SibA protein 			bind					IgG subclass 1					NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_8_4851_s_132	11447160	(Left) SibA protein immunoglobulin binding with IgG subclasses 1 to 4 and IgG antibody fragments.	bind
18491	2	5781	6	10	NULL	0	NULL	SibA protein			bind					IgG subclass 2					NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_8_4851_s_132	11447160	(Left) SibA protein immunoglobulin binding with IgG subclasses 1 to 4 and IgG antibody fragments.	bind
18492	3	5781	6	10	NULL	0	NULL	SibA protein			bind					IgG subclass 3					NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_8_4851_s_132	11447160	(Left) SibA protein immunoglobulin binding with IgG subclasses 1 to 4 and IgG antibody fragments.	bind
18493	4	5781	6	10	NULL	0	NULL	SibA protein			bind					IgG subclass 4					NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_8_4851_s_132	11447160	(Left) SibA protein immunoglobulin binding with IgG subclasses 1 to 4 and IgG antibody fragments.	bind
18494	5	5781	6	10	NULL	0	NULL	SibA protein	NULL		bind	NULL				IgG antibody fragments	NULL				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_8_4851_s_132	11447160	(Left) SibA protein immunoglobulin binding with IgG subclasses 1 to 4 and IgG antibody fragments.	bind
17633	1	5781	7	NULL	NULL	NULL	NULL	 SibA	GP		bind					IgG subclass 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_8_4851_s_132	11447160	(Left) SibA protein immunoglobulin binding with IgG subclasses 1 to 4 and IgG antibody fragments.	bind
17634	2	5781	7	NULL	NULL	NULL	NULL	SibA	GP		bind					IgG subclass 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_8_4851_s_132	11447160	(Left) SibA protein immunoglobulin binding with IgG subclasses 1 to 4 and IgG antibody fragments.	bind
17635	3	5781	7	NULL	NULL	NULL	NULL	SibA	GP		bind					IgG subclass 3	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_8_4851_s_132	11447160	(Left) SibA protein immunoglobulin binding with IgG subclasses 1 to 4 and IgG antibody fragments.	bind
17636	4	5781	7	NULL	NULL	NULL	NULL	SibA	GP		bind					IgG subclass 4	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_8_4851_s_132	11447160	(Left) SibA protein immunoglobulin binding with IgG subclasses 1 to 4 and IgG antibody fragments.	bind
17637	5	5781	7	NULL	NULL	NULL	NULL	SibA	GP		bind					IgG antibody fragments	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_8_4851_s_132	11447160	(Left) SibA protein immunoglobulin binding with IgG subclasses 1 to 4 and IgG antibody fragments.	bind
18495	1	5782	6	NULL	NULL	0	NULL	p300	NULL		bind	NULL				C/EBPbeta	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_1_472_s_301	15601867	(Lower panel)  Schematic representation of p300 showing the region that binds C/EBPbeta.	bind
17638	1	5782	7	NULL	NULL	NULL	NULL	p300	GP		bind					C/EBPbeta	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_1_472_s_301	15601867	(Lower panel)  Schematic representation of p300 showing the region that binds C/EBPbeta.	bind
18496	1	5783	6	10	NULL	0	NULL	Runx2	NULL	truncations	bind	NULL		N-108 series			NULL			Runx/octamer element	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3182_s_248	15798204	(Lower panel) EMSA showing binding of  the N-108 series of Runx2 truncations to the Runx/octamer element in the presence  or absence of Oct-1.	bind
17639	1	5783	7	NULL	NULL	NULL	NULL	Runx2	GP	truncations	bind			N-108 series						Runx/octamer element	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3182_s_248	15798204	(Lower panel) EMSA showing binding of  the N-108 series of Runx2 truncations to the Runx/octamer element in the presence  or absence of Oct-1.	bind
18497	1	5784	6	NULL	NULL	0	NULL	Nup116p	NULL		bind	NULL		GLEBS		Gle2p	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_17_4_1107_s_220	9463388	(Lower panel) Nup116p is drawn as a multi-domain protein which binds to Gle2p via its GLEBS and to importin/karyopherin beta-like transport factors (called beta-Kaps) via the GLFG region.	bind
18498	2	5784	6	NULL	NULL	0	NULL	Nup116p	NULL		bind	NULL		GLFG region		beta-Kaps	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_17_4_1107_s_220	9463388	(Lower panel) Nup116p is drawn as a multi-domain protein which binds to Gle2p via its GLEBS and to importin/karyopherin beta-like transport factors (called beta-Kaps) via the GLFG region.	bind
18499	3	5784	6	NULL	NULL	0	NULL	beta-Kaps	NULL		is	NULL				importin/karyopherin beta-like transport factors	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_17_4_1107_s_220	9463388	(Lower panel) Nup116p is drawn as a multi-domain protein which binds to Gle2p via its GLEBS and to importin/karyopherin beta-like transport factors (called beta-Kaps) via the GLFG region.	bind
17640	1	5784	7	NULL	NULL	NULL	NULL	Nup116p	GP		bind			GLEBS		Gle2p	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_4_1107_s_220	9463388	(Lower panel) Nup116p is drawn as a multi-domain protein which binds to Gle2p via its GLEBS and to importin/karyopherin beta-like transport factors (called beta-Kaps) via the GLFG region.	bind
17641	2	5784	7	NULL	NULL	NULL	NULL	Nup116p	GP		bind			GLFG region		beta-Kaps	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_4_1107_s_220	9463388	(Lower panel) Nup116p is drawn as a multi-domain protein which binds to Gle2p via its GLEBS and to importin/karyopherin beta-like transport factors (called beta-Kaps) via the GLFG region.	bind
17642	3	5784	7	NULL	NULL	NULL	NULL	importin/karyopherin beta-like transport factor	GP		is					beta-Kaps	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_4_1107_s_220	9463388	(Lower panel) Nup116p is drawn as a multi-domain protein which binds to Gle2p via its GLEBS and to importin/karyopherin beta-like transport factors (called beta-Kaps) via the GLFG region.	bind
18503	1	5785	6	NULL	NULL	0	NULL	IRP-1	NULL		bind	NULL					NULL			IRE	NULL		0	NULL	NULL	NULL	gw60_molcell_2_3_383_s_83	9774976	(Lower panel) The data presented in this manuscript reveal that translational inhibition by IRP-1 binding to the IRE permits eIF4F (eIF4E, eIF4G, and eIF4A) assembly but prevents the recruitment of eIF3/40S subunit complexes.	bind
18504	2	5785	6	10	NULL	0	NULL	statement 7	NULL		permits	NULL				eIF4F	NULL	assembly of 			NULL		NULL	NULL	NULL	NULL	gw60_molcell_2_3_383_s_83	9774976	(Lower panel) The data presented in this manuscript reveal that translational inhibition by IRP-1 binding to the IRE permits eIF4F (eIF4E, eIF4G, and eIF4A) assembly but prevents the recruitment of eIF3/40S subunit complexes.	bind
18511	3	5785	6	10	NULL	0	NULL	statement 7	NULL		prevents	NULL				eIF3/40S subunit complexes	NULL	recruitment of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_2_3_383_s_83	9774976	(Lower panel) The data presented in this manuscript reveal that translational inhibition by IRP-1 binding to the IRE permits eIF4F (eIF4E, eIF4G, and eIF4A) assembly but prevents the recruitment of eIF3/40S subunit complexes.	bind
53251	4	5785	6	10	NULL	0	NULL	eIF4F	NULL	assembly of	consists of	NULL				eIF4E	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_2_3_383_s_83	9774976	(Lower panel) The data presented in this manuscript reveal that translational inhibition by IRP-1 binding to the IRE permits eIF4F (eIF4E, eIF4G, and eIF4A) assembly but prevents the recruitment of eIF3/40S subunit complexes.	bind
53252	5	5785	6	10	NULL	0	NULL	eIF4F	NULL	assembly of	consists of	NULL				eIF4G	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_2_3_383_s_83	9774976	(Lower panel) The data presented in this manuscript reveal that translational inhibition by IRP-1 binding to the IRE permits eIF4F (eIF4E, eIF4G, and eIF4A) assembly but prevents the recruitment of eIF3/40S subunit complexes.	bind
53253	6	5785	6	10	NULL	0	NULL	eIF4F	NULL	assembly of	consists of	NULL				eIF4A	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcell_2_3_383_s_83	9774976	(Lower panel) The data presented in this manuscript reveal that translational inhibition by IRP-1 binding to the IRE permits eIF4F (eIF4E, eIF4G, and eIF4A) assembly but prevents the recruitment of eIF3/40S subunit complexes.	bind
53254	7	5785	6	10	NULL	0	NULL	statement 1	NULL		causes	NULL				translation	NULL	inhibition of			NULL		0	NULL	NULL	NULL	gw60_molcell_2_3_383_s_83	9774976	(Lower panel) The data presented in this manuscript reveal that translational inhibition by IRP-1 binding to the IRE permits eIF4F (eIF4E, eIF4G, and eIF4A) assembly but prevents the recruitment of eIF3/40S subunit complexes.	bind
17643	1	5785	7	NULL	NULL	NULL	NULL	IRP-1 	GP		bind									IRE	NULL		NULL	NULL	NULL	NULL	gw60_molcell_2_3_383_s_83	9774976	(Lower panel) The data presented in this manuscript reveal that translational inhibition by IRP-1 binding to the IRE permits eIF4F (eIF4E, eIF4G, and eIF4A) assembly but prevents the recruitment of eIF3/40S subunit complexes.	bind
17644	2	5785	7	NULL	NULL	NULL	NULL	statement 1	Process		cause					translation	Process	inhibition of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_2_3_383_s_83	9774976	(Lower panel) The data presented in this manuscript reveal that translational inhibition by IRP-1 binding to the IRE permits eIF4F (eIF4E, eIF4G, and eIF4A) assembly but prevents the recruitment of eIF3/40S subunit complexes.	bind
17645	3	5785	7	NULL	NULL	NULL	NULL	statement 2	Process		permits					eIF4F	GP	assembly of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_2_3_383_s_83	9774976	(Lower panel) The data presented in this manuscript reveal that translational inhibition by IRP-1 binding to the IRE permits eIF4F (eIF4E, eIF4G, and eIF4A) assembly but prevents the recruitment of eIF3/40S subunit complexes.	bind
17646	4	5785	7	NULL	NULL	NULL	NULL	eIF4F	GP	assembly of	consist of					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_2_3_383_s_83	9774976	(Lower panel) The data presented in this manuscript reveal that translational inhibition by IRP-1 binding to the IRE permits eIF4F (eIF4E, eIF4G, and eIF4A) assembly but prevents the recruitment of eIF3/40S subunit complexes.	bind
17647	5	5785	7	NULL	NULL	NULL	NULL	statement 2	Process		prevents					eIF3/40S subunit complex	GP	recruitment of 			NULL		NULL	NULL	NULL	NULL	gw60_molcell_2_3_383_s_83	9774976	(Lower panel) The data presented in this manuscript reveal that translational inhibition by IRP-1 binding to the IRE permits eIF4F (eIF4E, eIF4G, and eIF4A) assembly but prevents the recruitment of eIF3/40S subunit complexes.	bind
53249	6	5785	7	NULL	NULL	NULL	NULL	eIF4F	GP	assembly of	consists of					eIF4G	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_2_3_383_s_83	9774976	(Lower panel) The data presented in this manuscript reveal that translational inhibition by IRP-1 binding to the IRE permits eIF4F (eIF4E, eIF4G, and eIF4A) assembly but prevents the recruitment of eIF3/40S subunit complexes.	bind
53250	7	5785	7	NULL	NULL	NULL	NULL	eIF4F	GP	assembly of	consists of					eIF4A	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_2_3_383_s_83	9774976	(Lower panel) The data presented in this manuscript reveal that translational inhibition by IRP-1 binding to the IRE permits eIF4F (eIF4E, eIF4G, and eIF4A) assembly but prevents the recruitment of eIF3/40S subunit complexes.	bind
18512	1	5787	6	NULL	NULL	0	NULL	WER	NULL		regulates	NULL	positively			GL2	NULL	transcription of			NULL	heart stage embryos	0	NULL	NULL	NULL	gw60_development_130_13_2893_s_265	12756173	(Lower row)  WER positively regulates  GL2 transcription in heart stage embryos.	bind
17648	1	5787	7	NULL	NULL	NULL	NULL	WER	GP		regulates		positively			GL2	GP	transcription of			NULL	in heart stage embryos	NULL	NULL	NULL	NULL	gw60_development_130_13_2893_s_265	12756173	(Lower row)  WER positively regulates  GL2 transcription in heart stage embryos.	bind
18514	1	5788	6	10	NULL	0	NULL	COI	NULL		bind	NULL				M3	NULL				NULL	F1 mice immunized with B6 cells	NULL	NULL	NULL	NULL	gw70_annurevimmunol_15_0_851_s_63	9143709	(LP x B6)F1 mice immunized with B6 cells react to the  B6 form of COI presented by M3wt; so far, a response in the opposite direction has not been detected, although the  two forms of COI bind equally well to M3.	bind
17649	1	5788	7	NULL	NULL	NULL	NULL	COI	GP		bind					M3	GP				NULL	F1 mice immunized with B6 cells	NULL	NULL	NULL	NULL	gw70_annurevimmunol_15_0_851_s_63	9143709	(LP x B6)F1 mice immunized with B6 cells react to the  B6 form of COI presented by M3wt; so far, a response in the opposite direction has not been detected, although the  two forms of COI bind equally well to M3.	bind
18516	1	5791	6	NULL	NULL	0	NULL	Mdmx	NULL		bind	NULL		RING finger		Mdm2	NULL		RING finger		NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_70_0_503_s_383	11395416	(Mdmx and Mdm2 interact through their  RING fingers, which could prevent E2 binding to Mdm2.)	bind
18517	2	5791	6	NULL	NULL	0	NULL	E2	NULL		bind	NULL				Mdm2	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_70_0_503_s_383	11395416	(Mdmx and Mdm2 interact through their  RING fingers, which could prevent E2 binding to Mdm2.)	bind
18519	3	5791	6	NULL	NULL	0	NULL	statement 1	NULL		prevents	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_70_0_503_s_383	11395416	(Mdmx and Mdm2 interact through their  RING fingers, which could prevent E2 binding to Mdm2.)	bind
17821	1	5791	7	NULL	NULL	NULL	NULL	Mdmx	GP		bind			RING fingers		Mdm2	GP		RING fingers		NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_70_0_503_s_383	11395416	(Mdmx and Mdm2 interact through their  RING fingers, which could prevent E2 binding to Mdm2.)	bind
17822	2	5791	7	NULL	NULL	NULL	NULL	E2	GP		bind					Mdm2	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_70_0_503_s_383	11395416	(Mdmx and Mdm2 interact through their  RING fingers, which could prevent E2 binding to Mdm2.)	bind
17823	3	5791	7	NULL	NULL	NULL	NULL	statement 1	Process		prevents					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_70_0_503_s_383	11395416	(Mdmx and Mdm2 interact through their  RING fingers, which could prevent E2 binding to Mdm2.)	bind
18520	1	5793	6	NULL	NULL	0	NULL	HIC	NULL		bind	NULL				Axin	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_270	12192039	(Middle panel) HIC binding to Axin does not affect the binding of GSK-3beta, and the activation of JNK is decreased.	bind
18521	2	5793	6	NULL	NULL	0	NULL	statement 1	NULL		does not affect	NULL				GSK-3beta	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_270	12192039	(Middle panel) HIC binding to Axin does not affect the binding of GSK-3beta, and the activation of JNK is decreased.	bind
18525	3	5793	6	NULL	NULL	0	NULL	statement 1	NULL		decreases	NULL				JNK	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_270	12192039	(Middle panel) HIC binding to Axin does not affect the binding of GSK-3beta, and the activation of JNK is decreased.	bind
17824	1	5793	7	NULL	NULL	NULL	NULL	HIC	GP		bind					Axin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_270	12192039	(Middle panel) HIC binding to Axin does not affect the binding of GSK-3beta, and the activation of JNK is decreased.	bind
17825	2	5793	7	NULL	NULL	NULL	NULL	statement 1	Process		does not affect					GSK-3beta	Process	binding of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_270	12192039	(Middle panel) HIC binding to Axin does not affect the binding of GSK-3beta, and the activation of JNK is decreased.	bind
17826	3	5793	7	NULL	NULL	NULL	NULL	statement 1	Process		decrease					JNK	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_270	12192039	(Middle panel) HIC binding to Axin does not affect the binding of GSK-3beta, and the activation of JNK is decreased.	bind
18526	1	5795	6	10	NULL	0	NULL	Su(H)	NULL		bind	NULL	specifically				NULL			S1	NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_7_576_s_32	11937027	(N) The mobility-shift assay shows that Su(H) specifically binds to S1, S2, and S3.	bind
18527	2	5795	6	10	NULL	0	NULL	Su(H)	NULL		bind	NULL	specifically				NULL			S2	NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_7_576_s_32	11937027	(N) The mobility-shift assay shows that Su(H) specifically binds to S1, S2, and S3.	bind
18528	3	5795	6	10	NULL	0	NULL	Su(H)	NULL		bind	NULL	specifically				NULL			S3	NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_7_576_s_32	11937027	(N) The mobility-shift assay shows that Su(H) specifically binds to S1, S2, and S3.	bind
17827	1	5795	7	NULL	NULL	NULL	NULL	Su(H)	GP		binds		specifically							S1	NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_7_576_s_32	11937027	(N) The mobility-shift assay shows that Su(H) specifically binds to S1, S2, and S3.	bind
17828	2	5795	7	NULL	NULL	NULL	NULL	Su(H)	GP		binds		specifically							S2	NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_7_576_s_32	11937027	(N) The mobility-shift assay shows that Su(H) specifically binds to S1, S2, and S3.	bind
17829	3	5795	7	NULL	NULL	NULL	NULL	Su(H)	GP		binds		specifically							S3	NULL		NULL	NULL	NULL	NULL	gw60_currbiol_12_7_576_s_32	11937027	(N) The mobility-shift assay shows that Su(H) specifically binds to S1, S2, and S3.	bind
54105	1	5797	6	10	NULL	0	NULL	N3			bind		may;; directly			M2+					NULL		0	NULL	NULL	NULL	gw70_pnas_102_21_7459_s_10	15897459	(N3)H may possibly be acidified via carbonyl-coordinated M2+ to become a proton donor in the physiological pH range, at which direct (N3) -  binding of M2+ also seems possible.	bind
17830	1	5797	7	NULL	NULL	NULL	NULL	N3	Chemical		bind		may;;directly			M2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_21_7459_s_10	15897459	(N3)H may possibly be acidified via carbonyl-coordinated M2+ to become a proton donor in the physiological pH range, at which direct (N3) -  binding of M2+ also seems possible.	bind
18529	1	5798	6	10	NULL	0	NULL	StarD1	NULL	His-tagged;;full-length	bind	NULL	directly	START domain		cholesterol	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_46_8_1615_s_186	15897605	(N62)StarD1 and StarD5 containing START domains bind cholesterol   Tsujishita and Hurley ( ) reported data showing direct binding of cholesterol by a His-tagged StarD1 (full-length protein).	bind
18531	2	5798	6	10	NULL	0	NULL	StarD5	NULL		bind	NULL		START domain		cholesterol	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_46_8_1615_s_186	15897605	(N62)StarD1 and StarD5 containing START domains bind cholesterol   Tsujishita and Hurley ( ) reported data showing direct binding of cholesterol by a His-tagged StarD1 (full-length protein).	bind
17833	1	5798	7	NULL	NULL	NULL	NULL	StarD1	GP	His-tagged;;full-length	bind		directly	START domain		cholesterol	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_46_8_1615_s_186	15897605	(N62)StarD1 and StarD5 containing START domains bind cholesterol   Tsujishita and Hurley ( ) reported data showing direct binding of cholesterol by a His-tagged StarD1 (full-length protein).	bind
17834	2	5798	7	NULL	NULL	NULL	NULL	StarD5	GP		bind			START domain		cholesterol	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_46_8_1615_s_186	15897605	(N62)StarD1 and StarD5 containing START domains bind cholesterol   Tsujishita and Hurley ( ) reported data showing direct binding of cholesterol by a His-tagged StarD1 (full-length protein).	bind
24579	1	5800	6	10	NULL	0	NULL	ERK5	NULL		bind	NULL				deltakinase MEK5	NULL	mutant			NULL	cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_6_2065_s_122	16507987	(Nomenclature in the figures represents 64D65E-AA as 64.5DE-AA, etc.) (B) Binding of ERK5 and deltakinase MEK5 mutants in cells.	bind
12501	1	5800	7	NULL	NULL	NULL	NULL	ERK5	GP		bind					deltakinase MEK5 	GP	mutant			NULL	cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_6_2065_s_122	16507987	(Nomenclature in the figures represents 64D65E-AA as 64.5DE-AA, etc.) (B) Binding of ERK5 and deltakinase MEK5 mutants in cells.	bind
14894	1	5801	5	NULL	NULL	0	NULL	Annexin FITC	NULL		bind	NULL				mast cells	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_2_1439_s_191	11022038	(None) or with IL-3 or SCF (100 ng/ml) for 24 h. Annexin FITC binding to mast cells was determined by flow cytometry.	bind
17837	1	5801	7	NULL	NULL	NULL	NULL	 Annexin FITC	GP		bind					mast cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_2_1439_s_191	11022038	(None) or with IL-3 or SCF (100 ng/ml) for 24 h. Annexin FITC binding to mast cells was determined by flow cytometry.	bind
14895	1	5802	5	NULL	NULL	0	NULL	CFTR peptide	NULL		does not bind	NULL				beta2-syntrophin	NULL		PDZ domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_31_19797_s_124	9677412	(Not shown), we did not observe binding of the CFTR peptide to the PDZ domain of beta2-syntrophin (Fig.  4 B).	bind
17838	1	5802	7	NULL	NULL	NULL	NULL	CFTR peptide	GP		does not bind					beta2-syntrophin	GP		PDZ domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_31_19797_s_124	9677412	(Not shown), we did not observe binding of the CFTR peptide to the PDZ domain of beta2-syntrophin (Fig.  4 B).	bind
14896	1	5803	5	NULL	NULL	0	NULL	cytochrome c	NULL		bind	NULL				CCO	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_103_3_708_s_101	16407136	(Note that cytochrome   c is illustrated bound to CCO to denote the source of electrons, but this does not  imply cytochrome  c remains bound throughout multiple catalytic cycles.)	bind
17839	1	5803	7	NULL	NULL	NULL	NULL	cytochrome c 	GP		bind					CCO	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_3_708_s_101	16407136	(Note that cytochrome   c is illustrated bound to CCO to denote the source of electrons, but this does not  imply cytochrome  c remains bound throughout multiple catalytic cycles.)	bind
14897	1	5805	5	NULL	NULL	0	NULL	Pol II	NULL		bind	NULL					NULL			TATA region	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_13_5626_s_95	15964818	(Note that the ChIP signals for Pol II binding to the TATA region may be a composite of Pol II bound to the promoter and Pol II transcribing the 5' end of the ORF.)	bind
14898	2	5805	5	NULL	NULL	0	NULL	Pol II	NULL		bind	NULL					NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_13_5626_s_95	15964818	(Note that the ChIP signals for Pol II binding to the TATA region may be a composite of Pol II bound to the promoter and Pol II transcribing the 5' end of the ORF.)	bind
14899	3	5805	5	NULL	NULL	0	NULL	Pol II	NULL		transcribe	NULL					NULL			5' end of ORF	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_13_5626_s_95	15964818	(Note that the ChIP signals for Pol II binding to the TATA region may be a composite of Pol II bound to the promoter and Pol II transcribing the 5' end of the ORF.)	bind
14900	4	5805	5	NULL	NULL	0	NULL	statement 1	NULL		composite of 	NULL	may be			statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5626_s_95	15964818	(Note that the ChIP signals for Pol II binding to the TATA region may be a composite of Pol II bound to the promoter and Pol II transcribing the 5' end of the ORF.)	bind
14901	5	5805	5	NULL	NULL	0	NULL	statement 1	NULL		composite of	NULL	may be			statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5626_s_95	15964818	(Note that the ChIP signals for Pol II binding to the TATA region may be a composite of Pol II bound to the promoter and Pol II transcribing the 5' end of the ORF.)	bind
44720	6	5805	5	10	NULL	0	NULL	statement 2	NULL		occurs simultaneously with	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5626_s_95	15964818	(Note that the ChIP signals for Pol II binding to the TATA region may be a composite of Pol II bound to the promoter and Pol II transcribing the 5' end of the ORF.)	bind
17841	1	5805	7	NULL	NULL	NULL	NULL	Pol II	GP		bind									TATA region	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5626_s_95	15964818	(Note that the ChIP signals for Pol II binding to the TATA region may be a composite of Pol II bound to the promoter and Pol II transcribing the 5' end of the ORF.)	bind
17842	2	5805	7	NULL	NULL	NULL	NULL	Pol II	GP		bind									promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5626_s_95	15964818	(Note that the ChIP signals for Pol II binding to the TATA region may be a composite of Pol II bound to the promoter and Pol II transcribing the 5' end of the ORF.)	bind
17843	3	5805	7	NULL	NULL	NULL	NULL	Pol II	GP		transcribe									5' end of ORF	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5626_s_95	15964818	(Note that the ChIP signals for Pol II binding to the TATA region may be a composite of Pol II bound to the promoter and Pol II transcribing the 5' end of the ORF.)	bind
17844	4	5805	7	NULL	NULL	NULL	NULL	statement 2	Process		occur simultaneously with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5626_s_95	15964818	(Note that the ChIP signals for Pol II binding to the TATA region may be a composite of Pol II bound to the promoter and Pol II transcribing the 5' end of the ORF.)	bind
17845	5	5805	7	NULL	NULL	NULL	NULL	statement 1	Process		composite of		may be			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5626_s_95	15964818	(Note that the ChIP signals for Pol II binding to the TATA region may be a composite of Pol II bound to the promoter and Pol II transcribing the 5' end of the ORF.)	bind
17846	6	5805	7	NULL	NULL	NULL	NULL	statement 1	Process		composite of		may be			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5626_s_95	15964818	(Note that the ChIP signals for Pol II binding to the TATA region may be a composite of Pol II bound to the promoter and Pol II transcribing the 5' end of the ORF.)	bind
19164	1	5806	5	NULL	NULL	0	NULL	Rho protein	NULL		is the product of	NULL				rhomboid gene	NULL	Drosophila			NULL		0	NULL	NULL	NULL	gw60_genesdev_12_8_1166_s_26	9553046	(Note that the Rho protein described here is the product of  Drosophila gene  rhomboid, which bears no relationship with the mammalian membrane-bound GTPase Rho.)	bind
17848	1	5806	7	NULL	NULL	NULL	NULL	Rho protein	GP		is the product of					rhomboid gene	GP	Drosophila			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_8_1166_s_26	9553046	(Note that the Rho protein described here is the product of  Drosophila gene  rhomboid, which bears no relationship with the mammalian membrane-bound GTPase Rho.)	bind
14902	1	5807	5	NULL	NULL	0	NULL	SRF	NULL		bind	NULL				HDAC4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_22_20047_s_74	12663674	(Note that to assay the role of  Ca2+ on the binding of SRF and HDAC4, the basal protein interaction  buffer was altered by the addition of increasing concentrations of  Ca2+ (0 - 4 mM) or EGTA (10 mM).)	bind
19165	2	5807	5	NULL	NULL	0	NULL	Ca2+	NULL		has a role in	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_22_20047_s_74	12663674	(Note that to assay the role of  Ca2+ on the binding of SRF and HDAC4, the basal protein interaction  buffer was altered by the addition of increasing concentrations of  Ca2+ (0 - 4 mM) or EGTA (10 mM).)	bind
17849	1	5807	7	NULL	NULL	NULL	NULL	SRF	GP		bind					HDAC4	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_20047_s_74	12663674	(Note that to assay the role of  Ca2+ on the binding of SRF and HDAC4, the basal protein interaction  buffer was altered by the addition of increasing concentrations of  Ca2+ (0 - 4 mM) or EGTA (10 mM).)	bind
17850	2	5807	7	NULL	NULL	NULL	NULL	Ca2+	Chemical		has a role in					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_20047_s_74	12663674	(Note that to assay the role of  Ca2+ on the binding of SRF and HDAC4, the basal protein interaction  buffer was altered by the addition of increasing concentrations of  Ca2+ (0 - 4 mM) or EGTA (10 mM).)	bind
14903	1	5808	5	NULL	NULL	0	NULL	UV	NULL		induce	NULL				RNAP IIO	NULL	degradation of 			NULL		0	NULL	NULL	NULL	gw70_genesdev_19_10_1227_s_145	15905410	(Note that UV-induced degradation of RNAP IIO appeared somewhat greater when measured with H5, likely because H5 specifically recognizes the elongating form of RNAP II that would be targeted following UV.)	bind
14905	2	5808	5	10	NULL	0	NULL	H5	NULL		recognizes	NULL	specifically			RNAP II	NULL	elongating form of 			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_10_1227_s_145	15905410	(Note that UV-induced degradation of RNAP IIO appeared somewhat greater when measured with H5, likely because H5 specifically recognizes the elongating form of RNAP II that would be targeted following UV.)	bind
17851	1	5808	7	NULL	NULL	NULL	NULL	H5	GP		recognizes		specifically			RNAP II 	GP	elongating form of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_10_1227_s_145	15905410	(Note that UV-induced degradation of RNAP IIO appeared somewhat greater when measured with H5, likely because H5 specifically recognizes the elongating form of RNAP II that would be targeted following UV.)	bind
17852	2	5808	7	NULL	NULL	NULL	NULL	UV			induce					RNAP IIO	GP	degradation of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_10_1227_s_145	15905410	(Note that UV-induced degradation of RNAP IIO appeared somewhat greater when measured with H5, likely because H5 specifically recognizes the elongating form of RNAP II that would be targeted following UV.)	bind
14908	1	5810	5	10	NULL	0	NULL	cytidine	NULL		bind	NULL					NULL		cytidine binding site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_27_16962_s_275	9202008	(Note:  K2 is a stepwise macroscopic equilibrium constant; it corresponds to a microscopic constant for cytidine binding to the remaining cytidine binding site equal to 2.0 x 106M 1.)	bind
17853	1	5810	7	NULL	NULL	NULL	NULL	cytidine	Chemical		bind								cytidine binding site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_27_16962_s_275	9202008	(Note:  K2 is a stepwise macroscopic equilibrium constant; it corresponds to a microscopic constant for cytidine binding to the remaining cytidine binding site equal to 2.0 x 106M 1.)	bind
14911	1	5812	5	10	NULL	0	NULL	semaphorin-AP 	NULL		bind	NULL				neuropilin-expressing cells	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuron_19_3_547_s_81	9331348	(P-R) Equilibrium binding of semaphorin-AP fusion proteins to neuropilin-expressing cells.	bind
44779	2	5812	5	10	NULL	0	NULL	semaphorin-AP	NULL		is a type of	NULL				fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_19_3_547_s_81	9331348	(P-R) Equilibrium binding of semaphorin-AP fusion proteins to neuropilin-expressing cells.	bind
17854	1	5812	7	NULL	NULL	NULL	NULL	semaphorin-AP 	GP		bind					neuropilin-expressing cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_neuron_19_3_547_s_81	9331348	(P-R) Equilibrium binding of semaphorin-AP fusion proteins to neuropilin-expressing cells.	bind
44780	2	5812	7	NULL	NULL	NULL	NULL	semaphorin-AP	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_19_3_547_s_81	9331348	(P-R) Equilibrium binding of semaphorin-AP fusion proteins to neuropilin-expressing cells.	bind
14912	1	5814	5	10	NULL	0	NULL	p66shc	NULL		is a type of	NULL				splice variant of p52shc/p46shc	NULL				NULL		NULL	NULL	NULL	NULL	gw70_annurevgenomicshum_2_0_435_s_123	null	(p66shc is a splice variant of p52shc/p46shc, which binds Grb2 and may be involved  in Ras activation.)	bind
14913	2	5814	5	NULL	NULL	0	NULL	p66shc	NULL		bind	NULL				Grb2	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevgenomicshum_2_0_435_s_123	null	(p66shc is a splice variant of p52shc/p46shc, which binds Grb2 and may be involved  in Ras activation.)	bind
14914	3	5814	5	NULL	NULL	0	NULL	p66shc	NULL		involved in	NULL	may be			Ras	NULL	activation of			NULL		0	NULL	NULL	NULL	gw70_annurevgenomicshum_2_0_435_s_123	null	(p66shc is a splice variant of p52shc/p46shc, which binds Grb2 and may be involved  in Ras activation.)	bind
17857	1	5814	7	NULL	NULL	NULL	NULL	p66shc	GP		binds to					Grb2 	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevgenomicshum_2_0_435_s_123	null	(p66shc is a splice variant of p52shc/p46shc, which binds Grb2 and may be involved  in Ras activation.)	bind
17858	2	5814	7	NULL	NULL	NULL	NULL	p66shc	GP		 involved in		may be			Ras	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_annurevgenomicshum_2_0_435_s_123	null	(p66shc is a splice variant of p52shc/p46shc, which binds Grb2 and may be involved  in Ras activation.)	bind
17859	3	5814	7	NULL	NULL	NULL	NULL	p66shc	GP		is a type of					splice variant of p52shc/p46shc	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevgenomicshum_2_0_435_s_123	null	(p66shc is a splice variant of p52shc/p46shc, which binds Grb2 and may be involved  in Ras activation.)	bind
14915	1	5815	5	NULL	NULL	0	NULL	PABP-interacting protein 2	NULL		bind	NULL				PABP	NULL				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_rna_12_8_16804161_s_8	16804161	(PABP-interacting protein 2) binds PABP and inhibits  translation both in vitro and in vivo by decreasing the affinity of PABP  for polyadenylated RNA.	bind
14916	2	5815	5	NULL	NULL	0	NULL	PABP-interacting protein 2	NULL		inhibit	NULL				translation	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	abs-batch0740-0759_rna_12_8_16804161_s_8	16804161	(PABP-interacting protein 2) binds PABP and inhibits  translation both in vitro and in vivo by decreasing the affinity of PABP  for polyadenylated RNA.	bind
14917	3	5815	5	NULL	NULL	0	NULL	PABP-interacting protein 2	NULL		inhibit	NULL				translation	NULL				NULL	in vivo	0	NULL	NULL	NULL	abs-batch0740-0759_rna_12_8_16804161_s_8	16804161	(PABP-interacting protein 2) binds PABP and inhibits  translation both in vitro and in vivo by decreasing the affinity of PABP  for polyadenylated RNA.	bind
14918	4	5815	5	10	NULL	0	NULL	PABP			has affinity for					RNA		polyadenylated			NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_rna_12_8_16804161_s_8	16804161	(PABP-interacting protein 2) binds PABP and inhibits  translation both in vitro and in vivo by decreasing the affinity of PABP  for polyadenylated RNA.	bind
14919	5	5815	5	10	NULL	0	NULL	PABP-interacting protein 2	NULL		decrease	NULL				statement 4	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_rna_12_8_16804161_s_8	16804161	(PABP-interacting protein 2) binds PABP and inhibits  translation both in vitro and in vivo by decreasing the affinity of PABP  for polyadenylated RNA.	bind
14922	8	5815	5	NULL	NULL	0	NULL	statement 5	NULL		leads to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_rna_12_8_16804161_s_8	16804161	(PABP-interacting protein 2) binds PABP and inhibits  translation both in vitro and in vivo by decreasing the affinity of PABP  for polyadenylated RNA.	bind
14923	9	5815	5	NULL	NULL	0	NULL	statement 5	NULL		leads to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_rna_12_8_16804161_s_8	16804161	(PABP-interacting protein 2) binds PABP and inhibits  translation both in vitro and in vivo by decreasing the affinity of PABP  for polyadenylated RNA.	bind
17860	1	5815	7	NULL	NULL	NULL	NULL	PABP-interacting protein 2	GP		binds					PABP	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_rna_12_8_16804161_s_8	16804161	(PABP-interacting protein 2) binds PABP and inhibits  translation both in vitro and in vivo by decreasing the affinity of PABP  for polyadenylated RNA.	bind
17861	2	5815	7	NULL	NULL	NULL	NULL	statement 1	Process		inhibits					translation	Process				NULL	in vitro	NULL	NULL	NULL	NULL	abs-batch0740-0759_rna_12_8_16804161_s_8	16804161	(PABP-interacting protein 2) binds PABP and inhibits  translation both in vitro and in vivo by decreasing the affinity of PABP  for polyadenylated RNA.	bind
17862	3	5815	7	NULL	NULL	NULL	NULL	statement 1	Process		inhibits					translation	Process				NULL	in vivo	NULL	NULL	NULL	NULL	abs-batch0740-0759_rna_12_8_16804161_s_8	16804161	(PABP-interacting protein 2) binds PABP and inhibits  translation both in vitro and in vivo by decreasing the affinity of PABP  for polyadenylated RNA.	bind
17863	4	5815	7	NULL	NULL	NULL	NULL	PABP	GP		has affinity for					RNA	NucleicAcid	polyadenylated			NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_rna_12_8_16804161_s_8	16804161	(PABP-interacting protein 2) binds PABP and inhibits  translation both in vitro and in vivo by decreasing the affinity of PABP  for polyadenylated RNA.	bind
17864	5	5815	7	NULL	NULL	NULL	NULL	statement 1	Process		decreases					statement 4	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_rna_12_8_16804161_s_8	16804161	(PABP-interacting protein 2) binds PABP and inhibits  translation both in vitro and in vivo by decreasing the affinity of PABP  for polyadenylated RNA.	bind
17865	6	5815	7	NULL	NULL	NULL	NULL	statement 2	Process		occurs 					statement 5	Process	because of			NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_rna_12_8_16804161_s_8	16804161	(PABP-interacting protein 2) binds PABP and inhibits  translation both in vitro and in vivo by decreasing the affinity of PABP  for polyadenylated RNA.	bind
17866	7	5815	7	NULL	NULL	NULL	NULL	statement 3	Process		occurs 					statement 5	Process	because of			NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_rna_12_8_16804161_s_8	16804161	(PABP-interacting protein 2) binds PABP and inhibits  translation both in vitro and in vivo by decreasing the affinity of PABP  for polyadenylated RNA.	bind
14924	1	5816	5	NULL	NULL	0	NULL	GST	NULL	alone	does not bind	NULL	appreciably			TNNI3	NULL				NULL		0	NULL	NULL	NULL	gw70_gene_372_0_128_s_151	16516408	(Panel A), while GST alone does not appreciably bind  TNNI3.	bind
20289	1	5816	7	NULL	NULL	NULL	NULL	GST	Chemical		does not bind		appreciably			TNNI3	GP				NULL		NULL	NULL	NULL	NULL	gw70_gene_372_0_128_s_151	16516408	(Panel A), while GST alone does not appreciably bind  TNNI3.	bind
14925	1	5817	5	10	NULL	0	NULL	Polo-like		Xenopus	is required for					M-phase		exit of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7360_s_266	9819423	(Polo-like in  Xenopus) is required for M-phase exit and destruction of mitotic cyclins ( 5).	bind
14926	2	5817	5	10	NULL	0	NULL	Polo-like	NULL	Xenopus	is required for	NULL				mitotic cyclins	NULL	destruction of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7360_s_266	9819423	(Polo-like in  Xenopus) is required for M-phase exit and destruction of mitotic cyclins ( 5).	bind
17867	1	5817	7	NULL	NULL	NULL	NULL	Polo-like	OrganismPart	Xenopus	is required for					M-phase	Process	exit of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7360_s_266	9819423	(Polo-like in  Xenopus) is required for M-phase exit and destruction of mitotic cyclins ( 5).	bind
17868	2	5817	7	NULL	NULL	NULL	NULL	Polo-like	OrganismPart	Xenopus	is required for					mitotic cyclins	GP	destruction of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7360_s_266	9819423	(Polo-like in  Xenopus) is required for M-phase exit and destruction of mitotic cyclins ( 5).	bind
14927	1	5818	5	NULL	NULL	0	NULL	Ap 	NULL		bind	NULL		homeodomain		Ser wing	NULL			794 bp enhancer	NULL		0	NULL	NULL	NULL	gw70_development_131_2_285_s_194	14701680	(R-V) DNase I footprinting  analysis of the Ap homeodomain bound to the 794 bp  Ser wing enhancer.	bind
17869	1	5818	7	NULL	NULL	NULL	NULL	Ap	GP		bind			homeodomain		Ser wing	OrganismPart			 794 bp  enhancer	NULL		NULL	NULL	NULL	NULL	gw70_development_131_2_285_s_194	14701680	(R-V) DNase I footprinting  analysis of the Ap homeodomain bound to the 794 bp  Ser wing enhancer.	bind
14928	1	5819	5	10	NULL	0	NULL	Ap		HIS-tagged	bind		directly;;sequence specifically	homeodomain		Ser minimal wing				794 bp enhancer	NULL		NULL	NULL	NULL	NULL	gw70_development_131_2_285_s_193	14701680	(R-W) Binding of the Ap homeodomain (ApdeltaLIM, 6xHIS-tagged) to the 794 bp  Ser minimal wing enhancer is direct and sequence specific.	bind
54125	2	5819	5	10	NULL	0	NULL	Ap homeodomain			is					ApdeltaLIM					NULL		NULL	NULL	NULL	NULL	gw70_development_131_2_285_s_193	14701680	(R-W) Binding of the Ap homeodomain (ApdeltaLIM, 6xHIS-tagged) to the 794 bp  Ser minimal wing enhancer is direct and sequence specific.	bind
17870	1	5819	7	NULL	NULL	NULL	NULL	Ap	GP	HIS-tagged	binds		directly;;sequence specifically	homeodomain		Ser minimal wing	OrganismPart			794 bp enhancer	NULL		NULL	NULL	NULL	NULL	gw70_development_131_2_285_s_193	14701680	(R-W) Binding of the Ap homeodomain (ApdeltaLIM, 6xHIS-tagged) to the 794 bp  Ser minimal wing enhancer is direct and sequence specific.	bind
17872	2	5819	7	NULL	NULL	NULL	NULL	Ap homeodomain	GP		is					ApdeltaLIM	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_131_2_285_s_193	14701680	(R-W) Binding of the Ap homeodomain (ApdeltaLIM, 6xHIS-tagged) to the 794 bp  Ser minimal wing enhancer is direct and sequence specific.	bind
15610	1	5821	5	NULL	NULL	0	NULL	cyt P450	NULL	catalytic reaction of	involves	NULL				substrate 	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_35_36809_s_12	15194706	(REACTION 1) The cyt P450 catalytic reaction occurs via a reaction cycle that involves substrate binding, reduction of the ferric heme, O2 binding, reduction of the oxyferrous heme (second electron transfer), substrate oxidation, and finally product dissociation ( ).	bind
15611	2	5821	5	NULL	NULL	0	NULL	cyt P450	NULL	catalytic reaction of	involves	NULL				ferric heme	NULL	reduction of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_35_36809_s_12	15194706	(REACTION 1) The cyt P450 catalytic reaction occurs via a reaction cycle that involves substrate binding, reduction of the ferric heme, O2 binding, reduction of the oxyferrous heme (second electron transfer), substrate oxidation, and finally product dissociation ( ).	bind
15612	3	5821	5	NULL	NULL	0	NULL	cyt P450	NULL	catalytic reaction of	involves	NULL				O2	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_35_36809_s_12	15194706	(REACTION 1) The cyt P450 catalytic reaction occurs via a reaction cycle that involves substrate binding, reduction of the ferric heme, O2 binding, reduction of the oxyferrous heme (second electron transfer), substrate oxidation, and finally product dissociation ( ).	bind
15613	4	5821	5	NULL	NULL	0	NULL	cyt P450	NULL	catalytic reaction of	involves	NULL				oxyferrous heme	NULL	reduction of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_35_36809_s_12	15194706	(REACTION 1) The cyt P450 catalytic reaction occurs via a reaction cycle that involves substrate binding, reduction of the ferric heme, O2 binding, reduction of the oxyferrous heme (second electron transfer), substrate oxidation, and finally product dissociation ( ).	bind
15614	5	5821	5	NULL	NULL	0	NULL	cyt P450	NULL	catalytic reaction of	involves	NULL				substrate	NULL	oxidation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_35_36809_s_12	15194706	(REACTION 1) The cyt P450 catalytic reaction occurs via a reaction cycle that involves substrate binding, reduction of the ferric heme, O2 binding, reduction of the oxyferrous heme (second electron transfer), substrate oxidation, and finally product dissociation ( ).	bind
15615	6	5821	5	NULL	NULL	0	NULL	cyt P450	NULL	catalytic reaction of	involves	NULL				product	NULL	dissociation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_35_36809_s_12	15194706	(REACTION 1) The cyt P450 catalytic reaction occurs via a reaction cycle that involves substrate binding, reduction of the ferric heme, O2 binding, reduction of the oxyferrous heme (second electron transfer), substrate oxidation, and finally product dissociation ( ).	bind
17873	1	5821	7	NULL	NULL	NULL	NULL	cyt P450 	GP	catalytic reaction of	involves					substrate	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_35_36809_s_12	15194706	(REACTION 1) The cyt P450 catalytic reaction occurs via a reaction cycle that involves substrate binding, reduction of the ferric heme, O2 binding, reduction of the oxyferrous heme (second electron transfer), substrate oxidation, and finally product dissociation ( ).	bind
17874	2	5821	7	NULL	NULL	NULL	NULL	cyt P450 	GP	catalytic reaction of	involves					ferric heme	Chemical	reduction of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_35_36809_s_12	15194706	(REACTION 1) The cyt P450 catalytic reaction occurs via a reaction cycle that involves substrate binding, reduction of the ferric heme, O2 binding, reduction of the oxyferrous heme (second electron transfer), substrate oxidation, and finally product dissociation ( ).	bind
17875	3	5821	7	NULL	NULL	NULL	NULL	cyt P450	GP	catalytic reaction of	involves					O2	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_35_36809_s_12	15194706	(REACTION 1) The cyt P450 catalytic reaction occurs via a reaction cycle that involves substrate binding, reduction of the ferric heme, O2 binding, reduction of the oxyferrous heme (second electron transfer), substrate oxidation, and finally product dissociation ( ).	bind
17876	4	5821	7	NULL	NULL	NULL	NULL	cyt P450 	GP	catalytic reaction of	involves					oxyferrous heme	Chemical	reduction of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_35_36809_s_12	15194706	(REACTION 1) The cyt P450 catalytic reaction occurs via a reaction cycle that involves substrate binding, reduction of the ferric heme, O2 binding, reduction of the oxyferrous heme (second electron transfer), substrate oxidation, and finally product dissociation ( ).	bind
17877	5	5821	7	NULL	NULL	NULL	NULL	cyt P450 	GP	catalytic reaction of	involves					substrate	Chemical	oxidation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_35_36809_s_12	15194706	(REACTION 1) The cyt P450 catalytic reaction occurs via a reaction cycle that involves substrate binding, reduction of the ferric heme, O2 binding, reduction of the oxyferrous heme (second electron transfer), substrate oxidation, and finally product dissociation ( ).	bind
17878	6	5821	7	NULL	NULL	NULL	NULL	cyt P450 	Chemical	catalytic reaction of	involves					product	Chemical	dissociation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_35_36809_s_12	15194706	(REACTION 1) The cyt P450 catalytic reaction occurs via a reaction cycle that involves substrate binding, reduction of the ferric heme, O2 binding, reduction of the oxyferrous heme (second electron transfer), substrate oxidation, and finally product dissociation ( ).	bind
19166	1	5824	5	NULL	NULL	0	NULL	E7 peptide	NULL		bind	NULL		Leu			NULL		B-box helices		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_24_3199_s_206	12502741	(Red) Helices in B-box where the conserved Leu, Cys, and Glu in the E7 peptide bind; (magenta) helices from the other B-box in the asymmetric unit.	bind
19167	2	5824	5	NULL	NULL	0	NULL	E7 peptide	NULL		bind	NULL		Cys			NULL		B-box helices		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_24_3199_s_206	12502741	(Red) Helices in B-box where the conserved Leu, Cys, and Glu in the E7 peptide bind; (magenta) helices from the other B-box in the asymmetric unit.	bind
19168	3	5824	5	NULL	NULL	0	NULL	E7 peptide	NULL		bind	NULL		Glu			NULL		B-box helices		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_24_3199_s_206	12502741	(Red) Helices in B-box where the conserved Leu, Cys, and Glu in the E7 peptide bind; (magenta) helices from the other B-box in the asymmetric unit.	bind
17879	1	5824	7	NULL	NULL	NULL	NULL	E7 peptide	GP		bind			Leu					B-box helices		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_24_3199_s_206	12502741	(Red) Helices in B-box where the conserved Leu, Cys, and Glu in the E7 peptide bind; (magenta) helices from the other B-box in the asymmetric unit.	bind
17880	2	5824	7	NULL	NULL	NULL	NULL	E7 peptide	GP		bind			Cys					B-box helices		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_24_3199_s_206	12502741	(Red) Helices in B-box where the conserved Leu, Cys, and Glu in the E7 peptide bind; (magenta) helices from the other B-box in the asymmetric unit.	bind
17881	3	5824	7	NULL	NULL	NULL	NULL	E7 peptide	GP		bind			Glu					B-box helices		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_24_3199_s_206	12502741	(Red) Helices in B-box where the conserved Leu, Cys, and Glu in the E7 peptide bind; (magenta) helices from the other B-box in the asymmetric unit.	bind
14929	1	5825	5	NULL	NULL	0	NULL	Sox2	NULL		bind	NULL				FGF4	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_17_16_2048_s_25	12923055	(Remark: Sox2 binds  FGF4  and  UTF1 with similar affinity; see Supplemental Material.)	bind
14930	2	5825	5	NULL	NULL	0	NULL	Sox2	NULL		bind	NULL				UTF1	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_17_16_2048_s_25	12923055	(Remark: Sox2 binds  FGF4  and  UTF1 with similar affinity; see Supplemental Material.)	bind
14931	3	5825	5	10	NULL	0	NULL	statement 1	NULL		is similar to	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_16_2048_s_25	12923055	(Remark: Sox2 binds  FGF4  and  UTF1 with similar affinity; see Supplemental Material.)	bind
17882	1	5825	7	NULL	NULL	NULL	NULL	Sox2	GP		binds					FGF4	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_16_2048_s_25	12923055	(Remark: Sox2 binds  FGF4  and  UTF1 with similar affinity; see Supplemental Material.)	bind
17883	2	5825	7	NULL	NULL	NULL	NULL	Sox2	GP		binds					UTF1	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_16_2048_s_25	12923055	(Remark: Sox2 binds  FGF4  and  UTF1 with similar affinity; see Supplemental Material.)	bind
17884	3	5825	7	NULL	NULL	NULL	NULL	statement 1	Process		is similar to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_16_2048_s_25	12923055	(Remark: Sox2 binds  FGF4  and  UTF1 with similar affinity; see Supplemental Material.)	bind
14932	1	5827	5	NULL	NULL	0	NULL	cyclin D1	NULL		bind	NULL				cdk4	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3916_s_218	10207115	(Right panel) Inhibition of cyclin D1 binding to cdk4 on p16 induction.	bind
14933	2	5827	5	NULL	NULL	0	NULL	p16	NULL	induction	inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3916_s_218	10207115	(Right panel) Inhibition of cyclin D1 binding to cdk4 on p16 induction.	bind
17885	1	5827	7	NULL	NULL	NULL	NULL	cyclin D1	GP		bind					cdk4	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3916_s_218	10207115	(Right panel) Inhibition of cyclin D1 binding to cdk4 on p16 induction.	bind
17886	2	5827	7	NULL	NULL	NULL	NULL	p16	GP	induction of	inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3916_s_218	10207115	(Right panel) Inhibition of cyclin D1 binding to cdk4 on p16 induction.	bind
14934	1	5829	5	10	NULL	0	NULL	PACS-1	NULL		bind	NULL				TGN/endosomal proteins	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cell_94_2_205_s_76	9695949	(Right) Binding of PACS-1 to additional TGN/endosomal proteins.	bind
17887	1	5829	7	NULL	NULL	NULL	NULL	PACS-1	GP		bind					TGN/endosomal proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_94_2_205_s_76	9695949	(Right) Binding of PACS-1 to additional TGN/endosomal proteins.	bind
14935	1	5832	5	10	NULL	0	NULL	Munc13-1			bind					RIM1					NULL		NULL	NULL	NULL	NULL	gw60_neuron_30_1_183_s_116	11343654	(Right) Munc13-1 binding to RIM1-GST fusion proteins in cosedimentation assays.	bind
54126	2	5832	5	10	NULL	0	NULL	RIM1			is a type of					GST fusion protein					NULL		0	NULL	NULL	NULL	gw60_neuron_30_1_183_s_116	11343654	(Right) Munc13-1 binding to RIM1-GST fusion proteins in cosedimentation assays.	bind
17929	1	5832	7	NULL	NULL	NULL	NULL	Munc13-1	GP		bind					RIM1	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_30_1_183_s_116	11343654	(Right) Munc13-1 binding to RIM1-GST fusion proteins in cosedimentation assays.	bind
54127	2	5832	7	NULL	NULL	NULL	NULL	RIM1	GP		is a type of					GST fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_30_1_183_s_116	11343654	(Right) Munc13-1 binding to RIM1-GST fusion proteins in cosedimentation assays.	bind
14936	1	5833	5	NULL	NULL	0	NULL	Nt	NULL		bind	NULL				MTs	NULL				NULL		0	NULL	NULL	NULL	gw60_science_279_5350_580_s_48	9438855	(Right) Pellets containing Nt bound to MTs (Nt-MT complex) were incubated in the presence of 10 mM Mg-ATP, ultracentrifuged and analyzed as above.	bind
17933	1	5833	7	NULL	NULL	NULL	NULL	Nt	GP		bind					MTs	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_science_279_5350_580_s_48	9438855	(Right) Pellets containing Nt bound to MTs (Nt-MT complex) were incubated in the presence of 10 mM Mg-ATP, ultracentrifuged and analyzed as above.	bind
19169	1	5834	5	NULL	NULL	0	NULL	tRNA	NULL		bind	NULL					NULL		A-site		NULL		0	NULL	NULL	NULL	gw60_science_285_5434_1722_s_57	10481006	(Right) The graph shows quantification of interference of A-site tRNA binding by modification of N1 positions of A1492 and A1493.	bind
19170	2	5834	5	NULL	NULL	0	NULL		NULL	modification of	interferes with	NULL		N1 positions of A1492		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_science_285_5434_1722_s_57	10481006	(Right) The graph shows quantification of interference of A-site tRNA binding by modification of N1 positions of A1492 and A1493.	bind
19171	3	5834	5	NULL	NULL	0	NULL		NULL	modification of	interferes with	NULL		N1 positions of A1493		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_science_285_5434_1722_s_57	10481006	(Right) The graph shows quantification of interference of A-site tRNA binding by modification of N1 positions of A1492 and A1493.	bind
17937	1	5834	7	NULL	NULL	NULL	NULL	tRNA	NucleicAcid		binds								A-site		NULL		NULL	NULL	NULL	NULL	gw60_science_285_5434_1722_s_57	10481006	(Right) The graph shows quantification of interference of A-site tRNA binding by modification of N1 positions of A1492 and A1493.	bind
17938	2	5834	7	NULL	NULL	NULL	NULL			modification of	interferes with			N1 positions of A1492		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_285_5434_1722_s_57	10481006	(Right) The graph shows quantification of interference of A-site tRNA binding by modification of N1 positions of A1492 and A1493.	bind
17939	3	5834	7	NULL	NULL	NULL	NULL			modification of	interferes with			N1 positions of A1493		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_285_5434_1722_s_57	10481006	(Right) The graph shows quantification of interference of A-site tRNA binding by modification of N1 positions of A1492 and A1493.	bind
14937	1	5836	5	NULL	NULL	0	NULL	Bax	NULL		bind	NULL				PTP complex	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_155_5_695_s_29	11724809	(Right, PTP model) According to this model, Bax binds to the PTP complex and causes its opening, resulting in the swelling of the mitochondrial matrix and rupture of the OMM.	bind
14938	2	5836	5	NULL	NULL	0	NULL	statement 1	NULL		causes	NULL				PTP complex	NULL	opening of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_155_5_695_s_29	11724809	(Right, PTP model) According to this model, Bax binds to the PTP complex and causes its opening, resulting in the swelling of the mitochondrial matrix and rupture of the OMM.	bind
14939	3	5836	5	NULL	NULL	0	NULL	statement 2	NULL		results in	NULL				mitochondrial matrix	NULL	swelling of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_155_5_695_s_29	11724809	(Right, PTP model) According to this model, Bax binds to the PTP complex and causes its opening, resulting in the swelling of the mitochondrial matrix and rupture of the OMM.	bind
14940	4	5836	5	NULL	NULL	0	NULL	statement 2	NULL		results in	NULL				OMM	NULL	rupture of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_155_5_695_s_29	11724809	(Right, PTP model) According to this model, Bax binds to the PTP complex and causes its opening, resulting in the swelling of the mitochondrial matrix and rupture of the OMM.	bind
17947	1	5836	7	NULL	NULL	NULL	NULL	Bax 	GP		binds to					PTP complex 	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_5_695_s_29	11724809	(Right, PTP model) According to this model, Bax binds to the PTP complex and causes its opening, resulting in the swelling of the mitochondrial matrix and rupture of the OMM.	bind
17949	2	5836	7	NULL	NULL	NULL	NULL	statement 1	Process		cause					PTP complex 	GP	opening of			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_5_695_s_29	11724809	(Right, PTP model) According to this model, Bax binds to the PTP complex and causes its opening, resulting in the swelling of the mitochondrial matrix and rupture of the OMM.	bind
17951	3	5836	7	NULL	NULL	NULL	NULL	statement 1	Process		results in					mitochondrial matrix	CellComponent	swelling of			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_5_695_s_29	11724809	(Right, PTP model) According to this model, Bax binds to the PTP complex and causes its opening, resulting in the swelling of the mitochondrial matrix and rupture of the OMM.	bind
17952	4	5836	7	NULL	NULL	NULL	NULL	statement 1	Process		results in					OMM	CellComponent	rupture of			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_5_695_s_29	11724809	(Right, PTP model) According to this model, Bax binds to the PTP complex and causes its opening, resulting in the swelling of the mitochondrial matrix and rupture of the OMM.	bind
14941	1	5837	5	10	NULL	0	NULL	Sema IV AP 	NULL		bind	NULL				neuropilin-1- (S) expressing cells	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_6_1283_s_103	9883722	(S and T) Equilibrium binding of Sema IV AP fusion proteins to neuropilin-1- (S) or neuropilin-2- (T) expressing cells.	bind
14942	2	5837	5	10	NULL	0	NULL	Sema IV AP 	NULL		bind	NULL				neuropilin-2- (T) expressing cells	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_6_1283_s_103	9883722	(S and T) Equilibrium binding of Sema IV AP fusion proteins to neuropilin-1- (S) or neuropilin-2- (T) expressing cells.	bind
44781	3	5837	5	10	NULL	0	NULL	Sema IV AP	NULL		is a type of	NULL				fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_21_6_1283_s_103	9883722	(S and T) Equilibrium binding of Sema IV AP fusion proteins to neuropilin-1- (S) or neuropilin-2- (T) expressing cells.	bind
17969	1	5837	7	NULL	NULL	NULL	NULL	Sema IV AP	GP		bind					neuropilin-1- (S) expressing cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_6_1283_s_103	9883722	(S and T) Equilibrium binding of Sema IV AP fusion proteins to neuropilin-1- (S) or neuropilin-2- (T) expressing cells.	bind
17970	2	5837	7	NULL	NULL	NULL	NULL	Sema IV AP	GP		bind					neuropilin-2- (T) expressing cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_6_1283_s_103	9883722	(S and T) Equilibrium binding of Sema IV AP fusion proteins to neuropilin-1- (S) or neuropilin-2- (T) expressing cells.	bind
44782	3	5837	7	NULL	NULL	NULL	NULL	Sema IV AP	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_6_1283_s_103	9883722	(S and T) Equilibrium binding of Sema IV AP fusion proteins to neuropilin-1- (S) or neuropilin-2- (T) expressing cells.	bind
14943	1	5838	5	NULL	NULL	0	NULL	CAF	NULL		bind	NULL				TH	NULL				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_j-chromatogr-b-analyt-technol-biomed-life-sci_836_1-2_16621743_s_8	16621743	(Selectivity (alpha) is the ratio of  CAF bound to TH bound.)	bind
17971	1	5838	7	NULL	NULL	NULL	NULL	CAF	Chemical		bind					TH	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-chromatogr-b-analyt-technol-biomed-life-sci_836_1-2_16621743_s_8	16621743	(Selectivity (alpha) is the ratio of  CAF bound to TH bound.)	bind
19172	1	5839	5	10	NULL	0	NULL	sFRP/Frzb	NULL		bind	NULL	may			Fz proteins	NULL				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_276	11448771	(sFRP/Frzb may also bind certain Fz proteins, not depicted here).	bind
17973	1	5839	7	NULL	NULL	NULL	NULL	sFRP/Frzb	GP		bind		may			 Fz proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_11_12_951_s_276	11448771	(sFRP/Frzb may also bind certain Fz proteins, not depicted here).	bind
14944	1	5840	5	NULL	NULL	0	NULL	apo-B	NULL		bind	NULL				LDL receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_101_5_1084_s_39	9486979	(Site B) and developed a model that explains how sequences and mutations carboxyl-terminal to the  LDL receptor-binding site modulate the receptor-binding activity of apo-B for the LDL receptor.	bind
14945	2	5840	5	NULL	NULL	0	NULL		NULL	mutant	modulate	NULL		carboxyl-terminal to LDL receptor-binding site		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_101_5_1084_s_39	9486979	(Site B) and developed a model that explains how sequences and mutations carboxyl-terminal to the  LDL receptor-binding site modulate the receptor-binding activity of apo-B for the LDL receptor.	bind
17974	1	5840	7	NULL	NULL	NULL	NULL	apo-B	Chemical		bind					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_101_5_1084_s_39	9486979	(Site B) and developed a model that explains how sequences and mutations carboxyl-terminal to the  LDL receptor-binding site modulate the receptor-binding activity of apo-B for the LDL receptor.	bind
17975	2	5840	7	NULL	NULL	NULL	NULL			mutant	modulate			carboxyl-terminal to the LDL receptor-binding site 		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_101_5_1084_s_39	9486979	(Site B) and developed a model that explains how sequences and mutations carboxyl-terminal to the  LDL receptor-binding site modulate the receptor-binding activity of apo-B for the LDL receptor.	bind
14948	1	5843	5	NULL	NULL	0	NULL	PDK-1	NULL		bind	NULL				PIF	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_57_4_652_s_161	10727509	(Stephens et al., 1998  ), and also that binding of PIF to PDK-1 converts it into a PtdIns-3,4,5-P3-activated enzyme (Balendran et al., 1999a  ).	bind
14949	2	5843	5	NULL	NULL	0	NULL	statement 1	NULL		converted to	NULL				PtdIns-3,4,5-P3-activated enzyme	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_57_4_652_s_161	10727509	(Stephens et al., 1998  ), and also that binding of PIF to PDK-1 converts it into a PtdIns-3,4,5-P3-activated enzyme (Balendran et al., 1999a  ).	bind
17981	1	5843	7	NULL	NULL	NULL	NULL	PIF	GP		bind					PDK-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_57_4_652_s_161	10727509	(Stephens et al., 1998  ), and also that binding of PIF to PDK-1 converts it into a PtdIns-3,4,5-P3-activated enzyme (Balendran et al., 1999a  ).	bind
17982	2	5843	7	NULL	NULL	NULL	NULL	statement 1	Process		converts it to					PtdIns-3,4,5-P3-activated enzyme	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_57_4_652_s_161	10727509	(Stephens et al., 1998  ), and also that binding of PIF to PDK-1 converts it into a PtdIns-3,4,5-P3-activated enzyme (Balendran et al., 1999a  ).	bind
14969	1	5844	5	NULL	NULL	0	NULL	p53	NULL		bind	NULL	nonspecific			DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_10_8_2703_s_233	10436023	(Stimulations may be indirect: 14-3-3 may block nonspecific binding of p53 to DNA [ P16]; p300 may do the same consequential to acetylation of K382 [ P21,22].)	bind
14970	2	5844	5	NULL	NULL	0	NULL	14-3-3	NULL		blocks	NULL	may			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_10_8_2703_s_233	10436023	(Stimulations may be indirect: 14-3-3 may block nonspecific binding of p53 to DNA [ P16]; p300 may do the same consequential to acetylation of K382 [ P21,22].)	bind
17983	1	5844	7	NULL	NULL	NULL	NULL	p53	GP		bind		non-specifically			DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_8_2703_s_233	10436023	(Stimulations may be indirect: 14-3-3 may block nonspecific binding of p53 to DNA [ P16]; p300 may do the same consequential to acetylation of K382 [ P21,22].)	bind
17984	2	5844	7	NULL	NULL	NULL	NULL	14-3-3	Chemical		block		may			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_8_2703_s_233	10436023	(Stimulations may be indirect: 14-3-3 may block nonspecific binding of p53 to DNA [ P16]; p300 may do the same consequential to acetylation of K382 [ P21,22].)	bind
17987	1	5845	7	NULL	NULL	0	NULL	NADP+	NULL		bind	NULL				CL-DHFR	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1481_1_37_s_165	10962090	(Structure of NADP+-bound CL-DHFR was obtained from the Protein Data Bank, using the PDB accession code 8DFR.)	bind
14972	1	5846	5	NULL	NULL	0	NULL	ARG1	NULL		bind	NULL					NULL		myc-Arg81p		NULL		0	NULL	NULL	NULL	gw70_pnas_101_32_11713_s_128	15289616	(Student's  t test indicates that the reduction in  ARG1 binding of myc-Arg81p and myc-Arg82p produced by exogenous arginine is statistically significant, with  P values of 0.001 and 0.02, respectively.)	bind
14973	2	5846	5	NULL	NULL	0	NULL	ARG1	NULL		bind	NULL					NULL		myc-Arg82p		NULL		0	NULL	NULL	NULL	gw70_pnas_101_32_11713_s_128	15289616	(Student's  t test indicates that the reduction in  ARG1 binding of myc-Arg81p and myc-Arg82p produced by exogenous arginine is statistically significant, with  P values of 0.001 and 0.02, respectively.)	bind
14975	3	5846	5	NULL	NULL	0	NULL		NULL	exogenous	reduce	NULL		arginine		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_101_32_11713_s_128	15289616	(Student's  t test indicates that the reduction in  ARG1 binding of myc-Arg81p and myc-Arg82p produced by exogenous arginine is statistically significant, with  P values of 0.001 and 0.02, respectively.)	bind
14976	4	5846	5	NULL	NULL	0	NULL		NULL	exogenous	reduce	NULL		arginine		statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_101_32_11713_s_128	15289616	(Student's  t test indicates that the reduction in  ARG1 binding of myc-Arg81p and myc-Arg82p produced by exogenous arginine is statistically significant, with  P values of 0.001 and 0.02, respectively.)	bind
17988	1	5846	7	NULL	NULL	NULL	NULL	ARG1	AminoAcid		bind								myc-Arg81p		NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_32_11713_s_128	15289616	(Student's  t test indicates that the reduction in  ARG1 binding of myc-Arg81p and myc-Arg82p produced by exogenous arginine is statistically significant, with  P values of 0.001 and 0.02, respectively.)	bind
17989	2	5846	7	NULL	NULL	NULL	NULL	ARG1	AminoAcid		bind								myc-Arg82p		NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_32_11713_s_128	15289616	(Student's  t test indicates that the reduction in  ARG1 binding of myc-Arg81p and myc-Arg82p produced by exogenous arginine is statistically significant, with  P values of 0.001 and 0.02, respectively.)	bind
17990	3	5846	7	NULL	NULL	NULL	NULL	arginine	AminoAcid	exogenous	reduce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_32_11713_s_128	15289616	(Student's  t test indicates that the reduction in  ARG1 binding of myc-Arg81p and myc-Arg82p produced by exogenous arginine is statistically significant, with  P values of 0.001 and 0.02, respectively.)	bind
20290	4	5846	7	NULL	NULL	NULL	NULL	arginine	AminoAcid	exogenous	reduce					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_32_11713_s_128	15289616	(Student's  t test indicates that the reduction in  ARG1 binding of myc-Arg81p and myc-Arg82p produced by exogenous arginine is statistically significant, with  P values of 0.001 and 0.02, respectively.)	bind
14979	1	5847	5	NULL	NULL	0	NULL	SpoIIAA proteins	NULL		bind	NULL	noncovalent			SpoIIAB	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_12_3860_s_63	10368168	(Studies of noncovalent binding of the SpoIIAA proteins with SpoIIAB in the presence of ADP [ 1,  4] revealed no significant difference between SpoIIAA+, SpoIIAAG62D, and SpoIIAAG95D [results not shown.)	bind
14980	2	5847	5	NULL	NULL	0	NULL	statement 1	NULL		in the presence of	NULL				ADP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_12_3860_s_63	10368168	(Studies of noncovalent binding of the SpoIIAA proteins with SpoIIAB in the presence of ADP [ 1,  4] revealed no significant difference between SpoIIAA+, SpoIIAAG62D, and SpoIIAAG95D [results not shown.)	bind
17991	1	5847	7	NULL	NULL	NULL	NULL	SpoIIAA	GP		bind		noncovalently			SpoIIAB	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_12_3860_s_63	10368168	(Studies of noncovalent binding of the SpoIIAA proteins with SpoIIAB in the presence of ADP [ 1,  4] revealed no significant difference between SpoIIAA+, SpoIIAAG62D, and SpoIIAAG95D [results not shown.)	bind
20291	2	5847	7	NULL	NULL	NULL	NULL	statement 1	Process		in presence of					ADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_12_3860_s_63	10368168	(Studies of noncovalent binding of the SpoIIAA proteins with SpoIIAB in the presence of ADP [ 1,  4] revealed no significant difference between SpoIIAA+, SpoIIAAG62D, and SpoIIAAG95D [results not shown.)	bind
14981	1	5848	5	NULL	NULL	0	NULL	GTF3	NULL		bind	NULL				TnI SURE	NULL		BLM		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_24_8490_s_260	11713284	(SURE  827/ 808), confirming that GTF3 binds the TnI SURE via the BLM (lanes 18 to 21).	bind
17992	1	5848	7	NULL	NULL	NULL	NULL	GTF3	GP		binds					TnI SURE	GP		BLM		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_24_8490_s_260	11713284	(SURE  827/ 808), confirming that GTF3 binds the TnI SURE via the BLM (lanes 18 to 21).	bind
14983	1	5850	5	NULL	NULL	0	NULL	HRI	NULL		bind	NULL		N-terminal domain		heme	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_7_5171_s_258	10671563	(Table  I and Figs.  3 and  4) and that the N-terminal domain of HRI could bind heme (Fig.  8).	bind
17994	1	5850	7	NULL	NULL	NULL	NULL	HRI	GP		bind			N-terminal domain		heme	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_7_5171_s_258	10671563	(Table  I and Figs.  3 and  4) and that the N-terminal domain of HRI could bind heme (Fig.  8).	bind
14984	1	5851	5	NULL	NULL	0	NULL	importin 58	NULL		bind	NULL	poorly			T-ag	NULL		NLS		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_27_17191_s_57	9202041	(Table  I for T-ag sequences of the fusion proteins) using the dot blot technique indicated poor binding of importin 58 to the T-ag NLS in the absence of importin 97, which alone did not bind the T-ag NLS at all (Fig.  1 A).	bind
14985	2	5851	5	NULL	NULL	0	NULL	statement 1	NULL		in the absence of	NULL				importin 97	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_27_17191_s_57	9202041	(Table  I for T-ag sequences of the fusion proteins) using the dot blot technique indicated poor binding of importin 58 to the T-ag NLS in the absence of importin 97, which alone did not bind the T-ag NLS at all (Fig.  1 A).	bind
14986	3	5851	5	NULL	NULL	0	NULL	importin 97	NULL	alone	does not bind	NULL				T-ag	NULL		NLS		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_27_17191_s_57	9202041	(Table  I for T-ag sequences of the fusion proteins) using the dot blot technique indicated poor binding of importin 58 to the T-ag NLS in the absence of importin 97, which alone did not bind the T-ag NLS at all (Fig.  1 A).	bind
17995	1	5851	7	NULL	NULL	NULL	NULL	importin 58	GP		binds		poorly			T-ag	GP		NLS		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_27_17191_s_57	9202041	(Table  I for T-ag sequences of the fusion proteins) using the dot blot technique indicated poor binding of importin 58 to the T-ag NLS in the absence of importin 97, which alone did not bind the T-ag NLS at all (Fig.  1 A).	bind
17996	2	5851	7	NULL	NULL	NULL	NULL	importin 97	GP	alone	does not bind					T-ag	GP		NLS		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_27_17191_s_57	9202041	(Table  I for T-ag sequences of the fusion proteins) using the dot blot technique indicated poor binding of importin 58 to the T-ag NLS in the absence of importin 97, which alone did not bind the T-ag NLS at all (Fig.  1 A).	bind
20312	3	5851	7	NULL	NULL	NULL	NULL	statement 1	Process		 in the absence of					importin 97	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_27_17191_s_57	9202041	(Table  I for T-ag sequences of the fusion proteins) using the dot blot technique indicated poor binding of importin 58 to the T-ag NLS in the absence of importin 97, which alone did not bind the T-ag NLS at all (Fig.  1 A).	bind
14987	1	5852	5	NULL	NULL	0	NULL	mucin	NULL		bind	NULL				SLPI	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_22_13563_s_209	9593692	(Table  I) and mucin ( 35) bind to SLPI and, thus, might also be of physiologic importance.	bind
17997	1	5852	7	NULL	NULL	NULL	NULL	mucin	GP		bind					SLPI	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_22_13563_s_209	9593692	(Table  I) and mucin ( 35) bind to SLPI and, thus, might also be of physiologic importance.	bind
14988	1	5853	5	NULL	NULL	0	NULL	Oct-1	NULL		bind	NULL					NULL			betaA/T-rich element	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_43_30832_s_263	10521475	(Table  I) and the aforementioned A/T-rich elements, it is conceivable that Oct-1 binds the betaA/T-rich element under MOV conditions.	bind
14989	2	5853	5	NULL	NULL	0	NULL	statement 1	NULL		in the presence of	NULL				MOV conditions	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_43_30832_s_263	10521475	(Table  I) and the aforementioned A/T-rich elements, it is conceivable that Oct-1 binds the betaA/T-rich element under MOV conditions.	bind
17999	1	5853	7	NULL	NULL	NULL	NULL	Oct-1	GP		binds									 betaA/T-rich element	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_43_30832_s_263	10521475	(Table  I) and the aforementioned A/T-rich elements, it is conceivable that Oct-1 binds the betaA/T-rich element under MOV conditions.	bind
20313	2	5853	7	NULL	NULL	NULL	NULL	statement 1	Process		in the presence of					MOV conditions	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_43_30832_s_263	10521475	(Table  I) and the aforementioned A/T-rich elements, it is conceivable that Oct-1 binds the betaA/T-rich element under MOV conditions.	bind
14990	1	5854	5	NULL	NULL	0	NULL	DnaA	NULL		bind	NULL					NULL			oriV	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_25_17918_s_103	10364238	(Table  I) and the substantially reduced activity  in vitro (Fig.  2 A), suggesting that the function of DnaA box 4 is to initiate DnaA binding to  oriV.	bind
14991	2	5854	5	10	NULL	0	NULL	DnaA	NULL		initiates	NULL			box 4	statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17918_s_103	10364238	(Table  I) and the substantially reduced activity  in vitro (Fig.  2 A), suggesting that the function of DnaA box 4 is to initiate DnaA binding to  oriV.	bind
18000	1	5854	7	NULL	NULL	NULL	NULL	DnaA	NucleicAcid		binds									oriV	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17918_s_103	10364238	(Table  I) and the substantially reduced activity  in vitro (Fig.  2 A), suggesting that the function of DnaA box 4 is to initiate DnaA binding to  oriV.	bind
18001	2	5854	7	NULL	NULL	NULL	NULL	DnaA	NucleicAcid		initiates				box 4	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17918_s_103	10364238	(Table  I) and the substantially reduced activity  in vitro (Fig.  2 A), suggesting that the function of DnaA box 4 is to initiate DnaA binding to  oriV.	bind
14992	1	5855	5	NULL	NULL	0	NULL	VCAM-1	NULL	soluble	bind	NULL				VLA-4 	NULL	high affinity			NULL	on Lck-reconstituted cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_17_13891_s_208	11102438	(Table  I) and to the markedly higher binding of soluble VCAM-1 to high affinity VLA-4 on Lck-reconstituted cells, no significant difference was noted in the  koff of VLA-4 tethers mediated by the high or low affinity VLA-4 on Lck-reconstituted or Lck-deficient cells, respectively.	bind
18002	1	5855	7	NULL	NULL	NULL	NULL	VCAM-1	GP	soluble	bind					VLA-4 	GP	high affinity			NULL	Lck-reconstituted cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_17_13891_s_208	11102438	(Table  I) and to the markedly higher binding of soluble VCAM-1 to high affinity VLA-4 on Lck-reconstituted cells, no significant difference was noted in the  koff of VLA-4 tethers mediated by the high or low affinity VLA-4 on Lck-reconstituted or Lck-deficient cells, respectively.	bind
14993	1	5856	5	NULL	NULL	0	NULL	VIP	NULL	mutant	stimulate	NULL		H178A		cAMP	NULL	production of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_9_4990_s_147	9478946	(Table  I) and VIP-stimulated cAMP production (Fig.  2) observed for the H178A, H178D, and H178K mutants was not related to absence of expression at cell surface and was probably due to a drastic loss of intrinsic binding activity, contrasting with the constitutive activity and high VIP binding affinity of the H178R mutant.	bind
14997	2	5856	5	NULL	NULL	0	NULL	VIP	NULL	mutant	stimulate	NULL		H178D		cAMP	NULL	production of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_4990_s_147	9478946	(Table  I) and VIP-stimulated cAMP production (Fig.  2) observed for the H178A, H178D, and H178K mutants was not related to absence of expression at cell surface and was probably due to a drastic loss of intrinsic binding activity, contrasting with the constitutive activity and high VIP binding affinity of the H178R mutant.	bind
14998	3	5856	5	NULL	NULL	0	NULL	VIP	NULL	mutant	stimulate	NULL		H178K		cAMP	NULL	production of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_4990_s_147	9478946	(Table  I) and VIP-stimulated cAMP production (Fig.  2) observed for the H178A, H178D, and H178K mutants was not related to absence of expression at cell surface and was probably due to a drastic loss of intrinsic binding activity, contrasting with the constitutive activity and high VIP binding affinity of the H178R mutant.	bind
44783	4	5856	5	NULL	NULL	0	NULL	VIP	NULL		bind	NULL	high affinity				NULL	mutant	H178R		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_4990_s_147	9478946	(Table  I) and VIP-stimulated cAMP production (Fig.  2) observed for the H178A, H178D, and H178K mutants was not related to absence of expression at cell surface and was probably due to a drastic loss of intrinsic binding activity, contrasting with the constitutive activity and high VIP binding affinity of the H178R mutant.	bind
44784	5	5856	5	NULL	NULL	0	NULL	VIP	NULL		stimulate	NULL				cAMP	NULL	production of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_4990_s_147	9478946	(Table  I) and VIP-stimulated cAMP production (Fig.  2) observed for the H178A, H178D, and H178K mutants was not related to absence of expression at cell surface and was probably due to a drastic loss of intrinsic binding activity, contrasting with the constitutive activity and high VIP binding affinity of the H178R mutant.	bind
44785	6	5856	5	NULL	NULL	0	NULL	statement 1	NULL		occurs due to	NULL	probably			intrinsic binding activity	NULL	drastic loss of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_4990_s_147	9478946	(Table  I) and VIP-stimulated cAMP production (Fig.  2) observed for the H178A, H178D, and H178K mutants was not related to absence of expression at cell surface and was probably due to a drastic loss of intrinsic binding activity, contrasting with the constitutive activity and high VIP binding affinity of the H178R mutant.	bind
44786	7	5856	5	NULL	NULL	0	NULL	statement 2	NULL		occurs due to	NULL	probably			intrinsic binding activity	NULL	drastic loss of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_4990_s_147	9478946	(Table  I) and VIP-stimulated cAMP production (Fig.  2) observed for the H178A, H178D, and H178K mutants was not related to absence of expression at cell surface and was probably due to a drastic loss of intrinsic binding activity, contrasting with the constitutive activity and high VIP binding affinity of the H178R mutant.	bind
44787	8	5856	5	NULL	NULL	0	NULL	statement 3	NULL		occurs due to	NULL	probably			intrinsic binding activity	NULL	drastic loss of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_4990_s_147	9478946	(Table  I) and VIP-stimulated cAMP production (Fig.  2) observed for the H178A, H178D, and H178K mutants was not related to absence of expression at cell surface and was probably due to a drastic loss of intrinsic binding activity, contrasting with the constitutive activity and high VIP binding affinity of the H178R mutant.	bind
18003	1	5856	7	NULL	NULL	NULL	NULL	VIP	GP		stimulate					cAMP	Chemical	production of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_9_4990_s_147	9478946	(Table  I) and VIP-stimulated cAMP production (Fig.  2) observed for the H178A, H178D, and H178K mutants was not related to absence of expression at cell surface and was probably due to a drastic loss of intrinsic binding activity, contrasting with the constitutive activity and high VIP binding affinity of the H178R mutant.	bind
18004	2	5856	7	NULL	NULL	NULL	NULL	VIP	GP	mutant	stimulate			H178A		cAMP	Chemical	production of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_9_4990_s_147	9478946	(Table  I) and VIP-stimulated cAMP production (Fig.  2) observed for the H178A, H178D, and H178K mutants was not related to absence of expression at cell surface and was probably due to a drastic loss of intrinsic binding activity, contrasting with the constitutive activity and high VIP binding affinity of the H178R mutant.	bind
18005	3	5856	7	NULL	NULL	NULL	NULL	VIP	GP	mutant	stimulate			H178D		cAMP	Chemical	production of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_9_4990_s_147	9478946	(Table  I) and VIP-stimulated cAMP production (Fig.  2) observed for the H178A, H178D, and H178K mutants was not related to absence of expression at cell surface and was probably due to a drastic loss of intrinsic binding activity, contrasting with the constitutive activity and high VIP binding affinity of the H178R mutant.	bind
18006	4	5856	7	NULL	NULL	NULL	NULL	VIP	GP	mutant	stimulate			H178K		cAMP	Chemical	production of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_9_4990_s_147	9478946	(Table  I) and VIP-stimulated cAMP production (Fig.  2) observed for the H178A, H178D, and H178K mutants was not related to absence of expression at cell surface and was probably due to a drastic loss of intrinsic binding activity, contrasting with the constitutive activity and high VIP binding affinity of the H178R mutant.	bind
18008	5	5856	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs due to		probably			intrinsic binding activity	Process	drastic loss of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_9_4990_s_147	9478946	(Table  I) and VIP-stimulated cAMP production (Fig.  2) observed for the H178A, H178D, and H178K mutants was not related to absence of expression at cell surface and was probably due to a drastic loss of intrinsic binding activity, contrasting with the constitutive activity and high VIP binding affinity of the H178R mutant.	bind
18009	6	5856	7	NULL	NULL	NULL	NULL	VIP	GP		bind		high affinity					mutant	 H178R		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_9_4990_s_147	9478946	(Table  I) and VIP-stimulated cAMP production (Fig.  2) observed for the H178A, H178D, and H178K mutants was not related to absence of expression at cell surface and was probably due to a drastic loss of intrinsic binding activity, contrasting with the constitutive activity and high VIP binding affinity of the H178R mutant.	bind
14999	1	5857	5	NULL	NULL	0	NULL	ICAM-1 receptor	NULL		bind	NULL				rhinovirus	NULL	human			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_35_32294_s_232	12065582	(Table  I) are low and surprisingly similar to the binding of the ICAM-1 receptor to human rhinovirus ( 16).	bind
18011	1	5857	7	NULL	NULL	NULL	NULL	ICAM-1 receptor	GP		binds					rhinovirus	Organism	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_35_32294_s_232	12065582	(Table  I) are low and surprisingly similar to the binding of the ICAM-1 receptor to human rhinovirus ( 16).	bind
15000	1	5859	5	NULL	NULL	0	NULL	HSF	NULL		bind	NULL					NULL			HSE	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_50_32168_s_153	8943271	(Table  I) indicate that the first three complexes formed by HSF binding to an HSE contain, respectively, three, six, and nine HSF monomers per DNA molecule.	bind
15001	2	5859	5	NULL	NULL	0	NULL		NULL		contain	NULL			HSE	HSF monomers	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_50_32168_s_153	8943271	(Table  I) indicate that the first three complexes formed by HSF binding to an HSE contain, respectively, three, six, and nine HSF monomers per DNA molecule.	bind
18012	1	5859	7	NULL	NULL	NULL	NULL	HSF	GP		bind									HSE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_50_32168_s_153	8943271	(Table  I) indicate that the first three complexes formed by HSF binding to an HSE contain, respectively, three, six, and nine HSF monomers per DNA molecule.	bind
18015	2	5859	7	NULL	NULL	NULL	NULL				contain				HSE	 HSF monomers	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_50_32168_s_153	8943271	(Table  I) indicate that the first three complexes formed by HSF binding to an HSE contain, respectively, three, six, and nine HSF monomers per DNA molecule.	bind
15004	1	5860	5	NULL	NULL	0	NULL	NG2	NULL		bind	NULL				alpha2 (VI)	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_42_26110_s_129	8824254	(Table  I) indicate that the soluble alpha2 (VI) chain and type VI collagen effectively inhibit the binding of NG2 to alpha2 (VI)-coated wells, whereas the alpha1 (VI) chain and the N9-N2 (VI) chain slightly enhance this interaction.	bind
15005	2	5860	5	NULL	NULL	0	NULL	alpha2 (VI) chain	NULL	soluble	inhibit	NULL	effectively			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_42_26110_s_129	8824254	(Table  I) indicate that the soluble alpha2 (VI) chain and type VI collagen effectively inhibit the binding of NG2 to alpha2 (VI)-coated wells, whereas the alpha1 (VI) chain and the N9-N2 (VI) chain slightly enhance this interaction.	bind
15006	3	5860	5	NULL	NULL	0	NULL	type VI collagen	NULL		inhibit	NULL	efficiently			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_42_26110_s_129	8824254	(Table  I) indicate that the soluble alpha2 (VI) chain and type VI collagen effectively inhibit the binding of NG2 to alpha2 (VI)-coated wells, whereas the alpha1 (VI) chain and the N9-N2 (VI) chain slightly enhance this interaction.	bind
15007	4	5860	5	NULL	NULL	0	NULL	alpha1 (VI) chain	NULL		enhance	NULL	slightly			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_42_26110_s_129	8824254	(Table  I) indicate that the soluble alpha2 (VI) chain and type VI collagen effectively inhibit the binding of NG2 to alpha2 (VI)-coated wells, whereas the alpha1 (VI) chain and the N9-N2 (VI) chain slightly enhance this interaction.	bind
15008	5	5860	5	10	NULL	0	NULL		NULL		enhance	NULL	slightly	N9-N2 (VI) chain		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_42_26110_s_129	8824254	(Table  I) indicate that the soluble alpha2 (VI) chain and type VI collagen effectively inhibit the binding of NG2 to alpha2 (VI)-coated wells, whereas the alpha1 (VI) chain and the N9-N2 (VI) chain slightly enhance this interaction.	bind
18014	1	5860	7	NULL	NULL	NULL	NULL	NG2	Chemical		bind					alpha2 (VI)	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_42_26110_s_129	8824254	(Table  I) indicate that the soluble alpha2 (VI) chain and type VI collagen effectively inhibit the binding of NG2 to alpha2 (VI)-coated wells, whereas the alpha1 (VI) chain and the N9-N2 (VI) chain slightly enhance this interaction.	bind
18016	2	5860	7	NULL	NULL	NULL	NULL	alpha2 (VI) chain	GP	soluble	inhibit		effectively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_42_26110_s_129	8824254	(Table  I) indicate that the soluble alpha2 (VI) chain and type VI collagen effectively inhibit the binding of NG2 to alpha2 (VI)-coated wells, whereas the alpha1 (VI) chain and the N9-N2 (VI) chain slightly enhance this interaction.	bind
18017	3	5860	7	NULL	NULL	NULL	NULL	type VI collagen	GP		inhibit		effectively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_42_26110_s_129	8824254	(Table  I) indicate that the soluble alpha2 (VI) chain and type VI collagen effectively inhibit the binding of NG2 to alpha2 (VI)-coated wells, whereas the alpha1 (VI) chain and the N9-N2 (VI) chain slightly enhance this interaction.	bind
18018	4	5860	7	NULL	NULL	NULL	NULL	alpha1 (VI) chain	GP		enhance		slightly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_42_26110_s_129	8824254	(Table  I) indicate that the soluble alpha2 (VI) chain and type VI collagen effectively inhibit the binding of NG2 to alpha2 (VI)-coated wells, whereas the alpha1 (VI) chain and the N9-N2 (VI) chain slightly enhance this interaction.	bind
18019	5	5860	7	NULL	NULL	NULL	NULL				enhance		slightly	N9-N2 (VI) chain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_42_26110_s_129	8824254	(Table  I) indicate that the soluble alpha2 (VI) chain and type VI collagen effectively inhibit the binding of NG2 to alpha2 (VI)-coated wells, whereas the alpha1 (VI) chain and the N9-N2 (VI) chain slightly enhance this interaction.	bind
15011	1	5861	5	10	NULL	0	NULL	E-selectin	NULL		improves	NULL		region 4		HL-60 cell	NULL	binding activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_11_6254_s_80	9497351	(Table  I) indicate that when the three lysine residues of region 5 are present, E-selectin region 4 improves the HL-60 cell binding activity, whereas region 4 of P-selectin actually causes a loss of binding activity.	bind
15012	2	5861	5	NULL	NULL	0	NULL		NULL		is required for	NULL		three lysine residues of region 5		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_11_6254_s_80	9497351	(Table  I) indicate that when the three lysine residues of region 5 are present, E-selectin region 4 improves the HL-60 cell binding activity, whereas region 4 of P-selectin actually causes a loss of binding activity.	bind
15013	3	5861	5	10	NULL	0	NULL	P-selectin	NULL		causes	NULL		region 4		HL-60	NULL	loss of;; binding activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_11_6254_s_80	9497351	(Table  I) indicate that when the three lysine residues of region 5 are present, E-selectin region 4 improves the HL-60 cell binding activity, whereas region 4 of P-selectin actually causes a loss of binding activity.	bind
18020	1	5861	7	NULL	NULL	NULL	NULL	E-selectin	GP		improves			region 4		HL-60 cell	Cell	binding activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_11_6254_s_80	9497351	(Table  I) indicate that when the three lysine residues of region 5 are present, E-selectin region 4 improves the HL-60 cell binding activity, whereas region 4 of P-selectin actually causes a loss of binding activity.	bind
18021	2	5861	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs upon the presence of 								three lysine residues region 5		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_11_6254_s_80	9497351	(Table  I) indicate that when the three lysine residues of region 5 are present, E-selectin region 4 improves the HL-60 cell binding activity, whereas region 4 of P-selectin actually causes a loss of binding activity.	bind
18022	3	5861	7	NULL	NULL	NULL	NULL	P-selectin	GP		cause			region 4		HL-60 cell	Cell	loss of;; binding activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_11_6254_s_80	9497351	(Table  I) indicate that when the three lysine residues of region 5 are present, E-selectin region 4 improves the HL-60 cell binding activity, whereas region 4 of P-selectin actually causes a loss of binding activity.	bind
18023	4	5861	7	NULL	NULL	NULL	NULL	statement 3	Process		occurs upon the presence of								three lysine residues region 5		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_11_6254_s_80	9497351	(Table  I) indicate that when the three lysine residues of region 5 are present, E-selectin region 4 improves the HL-60 cell binding activity, whereas region 4 of P-selectin actually causes a loss of binding activity.	bind
15018	1	5862	5	10	NULL	0	NULL	polyene macrolide antibiotic			bind					membrane ergosterol					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_40_37855_s_127	12133835	(Table  I) or in the sensitivities to various agents such as amphotericin B, a polyene macrolide antibiotic that binds to membrane ergosterol and induces cellular leakage ( 34) (Fig.  1 B), detergents (SDS and Triton X-100), and ethanol (data not shown).	bind
15019	2	5862	5	NULL	NULL	0	NULL	statement 1	NULL		induce	NULL				cellular leakage	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_40_37855_s_127	12133835	(Table  I) or in the sensitivities to various agents such as amphotericin B, a polyene macrolide antibiotic that binds to membrane ergosterol and induces cellular leakage ( 34) (Fig.  1 B), detergents (SDS and Triton X-100), and ethanol (data not shown).	bind
18024	1	5862	7	NULL	NULL	NULL	NULL	polyene macrolide antibiotic	Chemical		binds to					membrane ergosterol	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_40_37855_s_127	12133835	(Table  I) or in the sensitivities to various agents such as amphotericin B, a polyene macrolide antibiotic that binds to membrane ergosterol and induces cellular leakage ( 34) (Fig.  1 B), detergents (SDS and Triton X-100), and ethanol (data not shown).	bind
18025	2	5862	7	NULL	NULL	NULL	NULL	statement 1	Process		induce					cellular leakage	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_40_37855_s_127	12133835	(Table  I) or in the sensitivities to various agents such as amphotericin B, a polyene macrolide antibiotic that binds to membrane ergosterol and induces cellular leakage ( 34) (Fig.  1 B), detergents (SDS and Triton X-100), and ethanol (data not shown).	bind
15021	1	5863	5	NULL	NULL	0	NULL	STAT3	NULL		bind	NULL				SIE probe	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_16_10723_s_149	10196143	(Table  I) or LIF-induced STAT3 binding to the SIE probe (data not shown).	bind
15022	2	5863	5	NULL	NULL	0	NULL	LIF	NULL		induce	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_16_10723_s_149	10196143	(Table  I) or LIF-induced STAT3 binding to the SIE probe (data not shown).	bind
18026	1	5863	7	NULL	NULL	NULL	NULL	STAT3	GP		bind					SIE probe	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_16_10723_s_149	10196143	(Table  I) or LIF-induced STAT3 binding to the SIE probe (data not shown).	bind
18027	2	5863	7	NULL	NULL	NULL	NULL	LIF	GP		induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_16_10723_s_149	10196143	(Table  I) or LIF-induced STAT3 binding to the SIE probe (data not shown).	bind
15023	1	5864	5	NULL	NULL	0	NULL	galanin	NULL		bind	NULL				GalR3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_51_31949_s_136	9405385	(Table  I) revealed that, like GalR2, Gly1 of galanin is not critical for galanin to bind GalR3, whereas this residue is important for binding of galanin to GalR1 ( 15).	bind
15024	2	5864	5	NULL	NULL	0	NULL	galanin	NULL		is not critical for	NULL		Gly1		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_51_31949_s_136	9405385	(Table  I) revealed that, like GalR2, Gly1 of galanin is not critical for galanin to bind GalR3, whereas this residue is important for binding of galanin to GalR1 ( 15).	bind
15025	3	5864	5	NULL	NULL	0	NULL	galanin	NULL		bind	NULL				GalR1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_51_31949_s_136	9405385	(Table  I) revealed that, like GalR2, Gly1 of galanin is not critical for galanin to bind GalR3, whereas this residue is important for binding of galanin to GalR1 ( 15).	bind
15026	4	5864	5	NULL	NULL	0	NULL	galanin	NULL		is important for	NULL		Gly1		statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_51_31949_s_136	9405385	(Table  I) revealed that, like GalR2, Gly1 of galanin is not critical for galanin to bind GalR3, whereas this residue is important for binding of galanin to GalR1 ( 15).	bind
18028	1	5864	7	NULL	NULL	NULL	NULL	galanin	GP		bind					GalR3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_31949_s_136	9405385	(Table  I) revealed that, like GalR2, Gly1 of galanin is not critical for galanin to bind GalR3, whereas this residue is important for binding of galanin to GalR1 ( 15).	bind
18029	2	5864	7	NULL	NULL	NULL	NULL	galanin	GP		bind					 GalR1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_31949_s_136	9405385	(Table  I) revealed that, like GalR2, Gly1 of galanin is not critical for galanin to bind GalR3, whereas this residue is important for binding of galanin to GalR1 ( 15).	bind
18030	3	5864	7	NULL	NULL	NULL	NULL	galanin	GP		is not critical for			Gly1		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_31949_s_136	9405385	(Table  I) revealed that, like GalR2, Gly1 of galanin is not critical for galanin to bind GalR3, whereas this residue is important for binding of galanin to GalR1 ( 15).	bind
18031	4	5864	7	NULL	NULL	NULL	NULL	galanin	GP		is important for			Gly1		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_31949_s_136	9405385	(Table  I) revealed that, like GalR2, Gly1 of galanin is not critical for galanin to bind GalR3, whereas this residue is important for binding of galanin to GalR1 ( 15).	bind
15027	1	5865	5	NULL	NULL	0	NULL	galactose	NULL		bind	NULL				WBA I	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_37_28483_s_136	10837488	(Table  I) than those involved in the binding of galactose with WBA I ( 10) and jacalin.	bind
15028	2	5865	5	NULL	NULL	0	NULL	galactose	NULL		bind	NULL				jacalin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_37_28483_s_136	10837488	(Table  I) than those involved in the binding of galactose with WBA I ( 10) and jacalin.	bind
18032	1	5865	7	NULL	NULL	NULL	NULL	galactose	Chemical		bind					WBA I	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_37_28483_s_136	10837488	(Table  I) than those involved in the binding of galactose with WBA I ( 10) and jacalin.	bind
18033	2	5865	7	NULL	NULL	NULL	NULL	galactose	Chemical		bind					jacalin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_37_28483_s_136	10837488	(Table  I) than those involved in the binding of galactose with WBA I ( 10) and jacalin.	bind
18034	1	5866	7	NULL	NULL	NULL	NULL	MHC I-binding peptide	GP	unextended 	chaperoned by					hsp70	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_20_17163_s_184	11278929	(Table  I) that (i) treatment with lactacystin inhibited re-presentation of all the  extended peptides, (ii) surprisingly, treatment of cells with lactacystin inhibited re-presentation of even the  precise unextended MHC I-binding peptides when chaperoned by hsp70 or hsp90; (iii) in another surprise, re-presentation of the precise MHC I binding peptide complexed to gp96 was not inhibited by lactacystin.	bind
18035	2	5866	7	NULL	NULL	NULL	NULL	MHC I-binding peptide	GP	unextended 	chaperoned by					hsp90	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_20_17163_s_184	11278929	(Table  I) that (i) treatment with lactacystin inhibited re-presentation of all the  extended peptides, (ii) surprisingly, treatment of cells with lactacystin inhibited re-presentation of even the  precise unextended MHC I-binding peptides when chaperoned by hsp70 or hsp90; (iii) in another surprise, re-presentation of the precise MHC I binding peptide complexed to gp96 was not inhibited by lactacystin.	bind
18036	3	5866	7	NULL	NULL	NULL	NULL	lactacystin	GP		inhibits					statement 1	Process	 re-presentation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_20_17163_s_184	11278929	(Table  I) that (i) treatment with lactacystin inhibited re-presentation of all the  extended peptides, (ii) surprisingly, treatment of cells with lactacystin inhibited re-presentation of even the  precise unextended MHC I-binding peptides when chaperoned by hsp70 or hsp90; (iii) in another surprise, re-presentation of the precise MHC I binding peptide complexed to gp96 was not inhibited by lactacystin.	bind
18037	4	5866	7	NULL	NULL	NULL	NULL	lactacystin	GP		inhibits					statement 2	Process	re-presentation of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_20_17163_s_184	11278929	(Table  I) that (i) treatment with lactacystin inhibited re-presentation of all the  extended peptides, (ii) surprisingly, treatment of cells with lactacystin inhibited re-presentation of even the  precise unextended MHC I-binding peptides when chaperoned by hsp70 or hsp90; (iii) in another surprise, re-presentation of the precise MHC I binding peptide complexed to gp96 was not inhibited by lactacystin.	bind
18038	5	5866	7	NULL	NULL	NULL	NULL	MHC I binding peptide	GP		forms complex with					gp96	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_20_17163_s_184	11278929	(Table  I) that (i) treatment with lactacystin inhibited re-presentation of all the  extended peptides, (ii) surprisingly, treatment of cells with lactacystin inhibited re-presentation of even the  precise unextended MHC I-binding peptides when chaperoned by hsp70 or hsp90; (iii) in another surprise, re-presentation of the precise MHC I binding peptide complexed to gp96 was not inhibited by lactacystin.	bind
18039	6	5866	7	NULL	NULL	NULL	NULL	lactacystin	GP		does not inhibit					statement 5	Process	re-presentation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_20_17163_s_184	11278929	(Table  I) that (i) treatment with lactacystin inhibited re-presentation of all the  extended peptides, (ii) surprisingly, treatment of cells with lactacystin inhibited re-presentation of even the  precise unextended MHC I-binding peptides when chaperoned by hsp70 or hsp90; (iii) in another surprise, re-presentation of the precise MHC I binding peptide complexed to gp96 was not inhibited by lactacystin.	bind
15029	1	5867	5	NULL	NULL	0	NULL	factor Xa	NULL		bind	NULL				PS membranes	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_8_5679_s_171	12438309	(Table  I) to that reported for factor Xa bound to PS membranes ( ), we see a 20-fold increase in rate because of adding factor Va to the PS membrane.	bind
15030	2	5867	5	NULL	NULL	0	NULL	factor Va	NULL		added to	NULL				PS membrane	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_5679_s_171	12438309	(Table  I) to that reported for factor Xa bound to PS membranes ( ), we see a 20-fold increase in rate because of adding factor Va to the PS membrane.	bind
20260	3	5867	5	NULL	NULL	0	NULL	statement 2	NULL		increases	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_8_5679_s_171	12438309	(Table  I) to that reported for factor Xa bound to PS membranes ( ), we see a 20-fold increase in rate because of adding factor Va to the PS membrane.	bind
18040	1	5867	7	NULL	NULL	NULL	NULL	 factor Xa	GP		bind					PS membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_5679_s_171	12438309	(Table  I) to that reported for factor Xa bound to PS membranes ( ), we see a 20-fold increase in rate because of adding factor Va to the PS membrane.	bind
18041	2	5867	7	NULL	NULL	NULL	NULL	factor Va	GP		added to					PS membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_5679_s_171	12438309	(Table  I) to that reported for factor Xa bound to PS membranes ( ), we see a 20-fold increase in rate because of adding factor Va to the PS membrane.	bind
18042	3	5867	7	NULL	NULL	NULL	NULL	statement 2	Process		increase					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_5679_s_171	12438309	(Table  I) to that reported for factor Xa bound to PS membranes ( ), we see a 20-fold increase in rate because of adding factor Va to the PS membrane.	bind
15031	1	5868	5	NULL	NULL	0	NULL	factor Xa	NULL		bind	NULL				PS membranes	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_8_5679_s_171	12438309	(Table  I) to that reported for factor Xa bound to PS membranes ( 2), we see a 20-fold increase in rate because of adding factor Va to the PS membrane.	bind
15032	2	5868	5	NULL	NULL	0	NULL	factor Va	NULL		added to	NULL				PS membrane	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_8_5679_s_171	12438309	(Table  I) to that reported for factor Xa bound to PS membranes ( 2), we see a 20-fold increase in rate because of adding factor Va to the PS membrane.	bind
20261	3	5868	5	NULL	NULL	0	NULL	statement 2	NULL		increases	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_8_5679_s_171	12438309	(Table  I) to that reported for factor Xa bound to PS membranes ( 2), we see a 20-fold increase in rate because of adding factor Va to the PS membrane.	bind
15035	1	5869	5	NULL	NULL	0	NULL	mAb	NULL		bind	NULL				G-CSF-R	NULL	WT			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_39_36779_s_134	11468284	(Table  I) were normalized with respect to level of receptor expression and level of binding of each mAb to WT G-CSF-R.	bind
18043	1	5869	7	NULL	NULL	NULL	NULL	mAb	GP		bind					G-CSF-R	GP	WT			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_39_36779_s_134	11468284	(Table  I) were normalized with respect to level of receptor expression and level of binding of each mAb to WT G-CSF-R.	bind
15036	1	5870	5	NULL	NULL	0	NULL	fragment B of PKC lambda	NULL		bind	NULL				FRS2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_27_19025_s_292	10383403	(Table  I) where only fragment B of PKC lambda binds to FRS2.	bind
18044	1	5870	7	NULL	NULL	NULL	NULL	fragment B PKC lambda	GP		binds to					FRS2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_27_19025_s_292	10383403	(Table  I) where only fragment B of PKC lambda binds to FRS2.	bind
15037	1	5871	5	NULL	NULL	0	NULL	H4B	NULL		bind	NULL					NULL	mutant	Trp-409		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_41_38280_s_200	11479310	(Table  I), and since we detect the same spectral changes induced by the binding of H4B to the Trp-409 mutants as those that we observed in the low frequency region upon binding of H4B to wild type nNOSox, we conclude that the structure of the heme pockets of the mutants is similar to that of the wild type enzyme.	bind
15038	2	5871	5	NULL	NULL	0	NULL	H4B	NULL		bind	NULL				nNOSox	NULL	wild-type			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_41_38280_s_200	11479310	(Table  I), and since we detect the same spectral changes induced by the binding of H4B to the Trp-409 mutants as those that we observed in the low frequency region upon binding of H4B to wild type nNOSox, we conclude that the structure of the heme pockets of the mutants is similar to that of the wild type enzyme.	bind
18045	1	5871	7	NULL	NULL	NULL	NULL	 H4B	GP		bind							mutant	Trp-409		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_41_38280_s_200	11479310	(Table  I), and since we detect the same spectral changes induced by the binding of H4B to the Trp-409 mutants as those that we observed in the low frequency region upon binding of H4B to wild type nNOSox, we conclude that the structure of the heme pockets of the mutants is similar to that of the wild type enzyme.	bind
18046	2	5871	7	NULL	NULL	NULL	NULL	H4B 	GP		bind					 nNOSox	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_41_38280_s_200	11479310	(Table  I), and since we detect the same spectral changes induced by the binding of H4B to the Trp-409 mutants as those that we observed in the low frequency region upon binding of H4B to wild type nNOSox, we conclude that the structure of the heme pockets of the mutants is similar to that of the wild type enzyme.	bind
15039	1	5872	5	NULL	NULL	0	NULL	GST-CtBP	NULL		bind	NULL				Ad12 E1A	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_33_20867_s_103	9694833	(Table  I), and the ability of each to inhibit the binding of GST-CtBP to Ad12 E1A was determined.	bind
18094	1	5872	7	NULL	NULL	NULL	NULL	GST-CtBP	GP		bind					 Ad12 E1A	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_33_20867_s_103	9694833	(Table  I), and the ability of each to inhibit the binding of GST-CtBP to Ad12 E1A was determined.	bind
15040	1	5873	5	NULL	NULL	0	NULL	growth factors	NULL		activate	NULL				SRF	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_43_30832_s_236	10521475	(Table  I), and the observations that the SRF is activated by growth factors, elevated levels of intracellular calcium, and mechanical stretch (three stimuli associated with MOV), we investigated whether the SRF might comprise a component of the enriched MOV-P binding activity.	bind
20336	2	5873	5	NULL	NULL	0	NULL	intracellular calcium	NULL	elevated levels of	activate	NULL				SRF	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_43_30832_s_236	10521475	(Table  I), and the observations that the SRF is activated by growth factors, elevated levels of intracellular calcium, and mechanical stretch (three stimuli associated with MOV), we investigated whether the SRF might comprise a component of the enriched MOV-P binding activity.	bind
20337	3	5873	5	NULL	NULL	0	NULL	mechanical stretch	NULL		activate	NULL				SRF	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_43_30832_s_236	10521475	(Table  I), and the observations that the SRF is activated by growth factors, elevated levels of intracellular calcium, and mechanical stretch (three stimuli associated with MOV), we investigated whether the SRF might comprise a component of the enriched MOV-P binding activity.	bind
18095	1	5873	7	NULL	NULL	NULL	NULL	growth factors	GP		activates					SRF	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_43_30832_s_236	10521475	(Table  I), and the observations that the SRF is activated by growth factors, elevated levels of intracellular calcium, and mechanical stretch (three stimuli associated with MOV), we investigated whether the SRF might comprise a component of the enriched MOV-P binding activity.	bind
18096	2	5873	7	NULL	NULL	NULL	NULL	intracellular calcium	Chemical	elevated levels of	activates					SRF	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_43_30832_s_236	10521475	(Table  I), and the observations that the SRF is activated by growth factors, elevated levels of intracellular calcium, and mechanical stretch (three stimuli associated with MOV), we investigated whether the SRF might comprise a component of the enriched MOV-P binding activity.	bind
20322	3	5873	7	NULL	NULL	NULL	NULL	mechanical stretch	Process		activates					SRF	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_43_30832_s_236	10521475	(Table  I), and the observations that the SRF is activated by growth factors, elevated levels of intracellular calcium, and mechanical stretch (three stimuli associated with MOV), we investigated whether the SRF might comprise a component of the enriched MOV-P binding activity.	bind
15041	1	5878	5	NULL	NULL	0	NULL	DnaA protein	NULL		bind	NULL				R4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_29_17035_s_150	8663334	(Table  I), DnaA protein bound to R4 with about 3-fold higher affinity than to R1 (Fig.  7).	bind
15042	2	5878	5	NULL	NULL	0	NULL	DnaA protein	NULL		bind	NULL				R1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_29_17035_s_150	8663334	(Table  I), DnaA protein bound to R4 with about 3-fold higher affinity than to R1 (Fig.  7).	bind
15043	3	5878	5	NULL	NULL	0	NULL	statement 1	NULL		has higher affinity than	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_29_17035_s_150	8663334	(Table  I), DnaA protein bound to R4 with about 3-fold higher affinity than to R1 (Fig.  7).	bind
18097	1	5878	7	NULL	NULL	NULL	NULL	DnaA protein	GP		bind					R4	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_29_17035_s_150	8663334	(Table  I), DnaA protein bound to R4 with about 3-fold higher affinity than to R1 (Fig.  7).	bind
18098	2	5878	7	NULL	NULL	NULL	NULL	DnaA protein	GP		bind					R1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_29_17035_s_150	8663334	(Table  I), DnaA protein bound to R4 with about 3-fold higher affinity than to R1 (Fig.  7).	bind
18099	3	5878	7	NULL	NULL	NULL	NULL	statement 1	Process		has higher affinity than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_29_17035_s_150	8663334	(Table  I), DnaA protein bound to R4 with about 3-fold higher affinity than to R1 (Fig.  7).	bind
15044	1	5879	5	NULL	NULL	0	NULL	peptide inhibitor	NULL		bind	NULL				IKKbeta	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_46_32655_s_238	10551820	(Table  I), indicating that the binding of the peptide inhibitor to IKKbeta has no effect on the affinity for ATP.	bind
15045	2	5879	5	NULL	NULL	0	NULL	statement 1	NULL		does not effect	NULL				ATP	NULL	affinity for 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_46_32655_s_238	10551820	(Table  I), indicating that the binding of the peptide inhibitor to IKKbeta has no effect on the affinity for ATP.	bind
18100	1	5879	7	NULL	NULL	NULL	NULL	peptide inhibitor	GP		bind					IKKbeta	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_46_32655_s_238	10551820	(Table  I), indicating that the binding of the peptide inhibitor to IKKbeta has no effect on the affinity for ATP.	bind
18101	2	5879	7	NULL	NULL	NULL	NULL	statement 1	Process		has no affinity for					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_46_32655_s_238	10551820	(Table  I), indicating that the binding of the peptide inhibitor to IKKbeta has no effect on the affinity for ATP.	bind
15279	1	5880	5	NULL	NULL	0	NULL	vWf	NULL		bind	NULL				collagen	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_18_12300_s_238	10212199	(Table  I), indicating that the rate of association of factor VIII with vWf is not significantly affected after vWf binds to collagen.	bind
15280	2	5880	5	NULL	NULL	0	NULL	factor VIII	NULL		associate with	NULL				vWf	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_18_12300_s_238	10212199	(Table  I), indicating that the rate of association of factor VIII with vWf is not significantly affected after vWf binds to collagen.	bind
15281	3	5880	5	10	NULL	0	NULL	statement 2	NULL		does not affect	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_18_12300_s_238	10212199	(Table  I), indicating that the rate of association of factor VIII with vWf is not significantly affected after vWf binds to collagen.	bind
18102	1	5880	7	NULL	NULL	NULL	NULL	 factor VIII 	GP		bind					vWf	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_18_12300_s_238	10212199	(Table  I), indicating that the rate of association of factor VIII with vWf is not significantly affected after vWf binds to collagen.	bind
18103	2	5880	7	NULL	NULL	NULL	NULL	 vWf	GP		binds to					collagen	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_18_12300_s_238	10212199	(Table  I), indicating that the rate of association of factor VIII with vWf is not significantly affected after vWf binds to collagen.	bind
18104	3	5880	7	NULL	NULL	NULL	NULL	statement 1	Process		does not affect					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_18_12300_s_238	10212199	(Table  I), indicating that the rate of association of factor VIII with vWf is not significantly affected after vWf binds to collagen.	bind
15282	1	5881	5	NULL	NULL	0	NULL	IRS 3	NULL		does not bind	NULL				FKHR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_14_11782_s_269	12556524	(Table  I), its expression was still not induced by FKHR overexpression (Fig.  5), suggesting that IRS 3 cannot bind FKHR even when multimerized.	bind
15283	2	5881	5	NULL	NULL	0	NULL	IRS 3	NULL	multimerized	does not bind	NULL				FKHR	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_14_11782_s_269	12556524	(Table  I), its expression was still not induced by FKHR overexpression (Fig.  5), suggesting that IRS 3 cannot bind FKHR even when multimerized.	bind
18105	1	5881	7	NULL	NULL	NULL	NULL	IRS 3	GP		does not bind					FKHR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_14_11782_s_269	12556524	(Table  I), its expression was still not induced by FKHR overexpression (Fig.  5), suggesting that IRS 3 cannot bind FKHR even when multimerized.	bind
18106	2	5881	7	NULL	NULL	NULL	NULL	IRS 3	GP	multimerized 	does not bind					FKHR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_14_11782_s_269	12556524	(Table  I), its expression was still not induced by FKHR overexpression (Fig.  5), suggesting that IRS 3 cannot bind FKHR even when multimerized.	bind
15289	1	5883	5	NULL	NULL	0	NULL	PABA	NULL		bind	NULL				FXa	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_47_36876_s_359	10973949	(Table  I), PABA (Table  II), or TFPI (Table  III) binding to FXa ~4.5-fold.	bind
15290	2	5883	5	NULL	NULL	0	NULL	TFPI	NULL		bind	NULL				FXa	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_47_36876_s_359	10973949	(Table  I), PABA (Table  II), or TFPI (Table  III) binding to FXa ~4.5-fold.	bind
18110	1	5883	7	NULL	NULL	NULL	NULL	PABA	Chemical		bind					FXa	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_47_36876_s_359	10973949	(Table  I), PABA (Table  II), or TFPI (Table  III) binding to FXa ~4.5-fold.	bind
18111	2	5883	7	NULL	NULL	NULL	NULL	TFPI	GP		bind					FXa	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_47_36876_s_359	10973949	(Table  I), PABA (Table  II), or TFPI (Table  III) binding to FXa ~4.5-fold.	bind
15322	1	5884	5	NULL	NULL	0	NULL	G-CSF	NULL	mutant	bind	NULL		K23A		GR	NULL		R288A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17445_s_108	10364174	(Table  I), the mutant/WT ratios of the binding affinity of K23A, E46A, and D112A G-CSFs to (R288A)GR were greater than the corresponding ratios with WT-GR, suggesting a synergistic effect of receptor and G-CSF mutations.	bind
15324	2	5884	5	NULL	NULL	0	NULL	G-CSF	NULL	mutant	bind	NULL		E46A		GR	NULL		R288A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17445_s_108	10364174	(Table  I), the mutant/WT ratios of the binding affinity of K23A, E46A, and D112A G-CSFs to (R288A)GR were greater than the corresponding ratios with WT-GR, suggesting a synergistic effect of receptor and G-CSF mutations.	bind
15326	3	5884	5	NULL	NULL	0	NULL	G-CSF	NULL	mutant	bind	NULL		D112A		GR	NULL		R288A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17445_s_108	10364174	(Table  I), the mutant/WT ratios of the binding affinity of K23A, E46A, and D112A G-CSFs to (R288A)GR were greater than the corresponding ratios with WT-GR, suggesting a synergistic effect of receptor and G-CSF mutations.	bind
44834	4	5884	5	NULL	NULL	0	NULL	G-CSF	NULL	mutant	bind	NULL		K23A		GR	NULL	WT			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_25_17445_s_108	10364174	(Table  I), the mutant/WT ratios of the binding affinity of K23A, E46A, and D112A G-CSFs to (R288A)GR were greater than the corresponding ratios with WT-GR, suggesting a synergistic effect of receptor and G-CSF mutations.	bind
44835	5	5884	5	NULL	NULL	0	NULL	G-CSF	NULL	mutant	bind	NULL		E46A		GR	NULL	WT			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_25_17445_s_108	10364174	(Table  I), the mutant/WT ratios of the binding affinity of K23A, E46A, and D112A G-CSFs to (R288A)GR were greater than the corresponding ratios with WT-GR, suggesting a synergistic effect of receptor and G-CSF mutations.	bind
44836	6	5884	5	NULL	NULL	0	NULL	G-CSF	NULL	mutant	bind	NULL		D112A		GR	NULL	WT			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_25_17445_s_108	10364174	(Table  I), the mutant/WT ratios of the binding affinity of K23A, E46A, and D112A G-CSFs to (R288A)GR were greater than the corresponding ratios with WT-GR, suggesting a synergistic effect of receptor and G-CSF mutations.	bind
44837	7	5884	5	NULL	NULL	0	NULL	statement 1	NULL		greater than	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_25_17445_s_108	10364174	(Table  I), the mutant/WT ratios of the binding affinity of K23A, E46A, and D112A G-CSFs to (R288A)GR were greater than the corresponding ratios with WT-GR, suggesting a synergistic effect of receptor and G-CSF mutations.	bind
44838	8	5884	5	NULL	NULL	0	NULL	statement 2	NULL		greater than	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_25_17445_s_108	10364174	(Table  I), the mutant/WT ratios of the binding affinity of K23A, E46A, and D112A G-CSFs to (R288A)GR were greater than the corresponding ratios with WT-GR, suggesting a synergistic effect of receptor and G-CSF mutations.	bind
44839	9	5884	5	NULL	NULL	0	NULL	statement 3	NULL		greater than	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_25_17445_s_108	10364174	(Table  I), the mutant/WT ratios of the binding affinity of K23A, E46A, and D112A G-CSFs to (R288A)GR were greater than the corresponding ratios with WT-GR, suggesting a synergistic effect of receptor and G-CSF mutations.	bind
18112	1	5884	7	NULL	NULL	NULL	NULL	G-CSF	GP	mutant	bind 			K23A		GR	GP		R288A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17445_s_108	10364174	(Table  I), the mutant/WT ratios of the binding affinity of K23A, E46A, and D112A G-CSFs to (R288A)GR were greater than the corresponding ratios with WT-GR, suggesting a synergistic effect of receptor and G-CSF mutations.	bind
18113	2	5884	7	NULL	NULL	NULL	NULL	G-CSF	GP	mutant	bind			E46A		GR	GP		R288A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17445_s_108	10364174	(Table  I), the mutant/WT ratios of the binding affinity of K23A, E46A, and D112A G-CSFs to (R288A)GR were greater than the corresponding ratios with WT-GR, suggesting a synergistic effect of receptor and G-CSF mutations.	bind
18114	3	5884	7	NULL	NULL	NULL	NULL	G-CSF	GP	mutant	bind			D112A		GR	GP		R288A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17445_s_108	10364174	(Table  I), the mutant/WT ratios of the binding affinity of K23A, E46A, and D112A G-CSFs to (R288A)GR were greater than the corresponding ratios with WT-GR, suggesting a synergistic effect of receptor and G-CSF mutations.	bind
18115	4	5884	7	NULL	NULL	NULL	NULL	G-CSF	GP	mutant	bind			K23A		GR	GP	WT			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17445_s_108	10364174	(Table  I), the mutant/WT ratios of the binding affinity of K23A, E46A, and D112A G-CSFs to (R288A)GR were greater than the corresponding ratios with WT-GR, suggesting a synergistic effect of receptor and G-CSF mutations.	bind
18116	5	5884	7	NULL	NULL	NULL	NULL	G-CSF	GP	mutant	bind			E46A		GR	GP	WT			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17445_s_108	10364174	(Table  I), the mutant/WT ratios of the binding affinity of K23A, E46A, and D112A G-CSFs to (R288A)GR were greater than the corresponding ratios with WT-GR, suggesting a synergistic effect of receptor and G-CSF mutations.	bind
18117	6	5884	7	NULL	NULL	NULL	NULL	G-CSF	GP	mutant	bind			D112A 		GR	GP	WT			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17445_s_108	10364174	(Table  I), the mutant/WT ratios of the binding affinity of K23A, E46A, and D112A G-CSFs to (R288A)GR were greater than the corresponding ratios with WT-GR, suggesting a synergistic effect of receptor and G-CSF mutations.	bind
18118	7	5884	7	NULL	NULL	NULL	NULL	statement 1	Process		is greater than					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17445_s_108	10364174	(Table  I), the mutant/WT ratios of the binding affinity of K23A, E46A, and D112A G-CSFs to (R288A)GR were greater than the corresponding ratios with WT-GR, suggesting a synergistic effect of receptor and G-CSF mutations.	bind
18119	8	5884	7	NULL	NULL	NULL	NULL	statement 2	Process		is greater than					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17445_s_108	10364174	(Table  I), the mutant/WT ratios of the binding affinity of K23A, E46A, and D112A G-CSFs to (R288A)GR were greater than the corresponding ratios with WT-GR, suggesting a synergistic effect of receptor and G-CSF mutations.	bind
18120	9	5884	7	NULL	NULL	NULL	NULL	statement 3	Process		is greater than					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17445_s_108	10364174	(Table  I), the mutant/WT ratios of the binding affinity of K23A, E46A, and D112A G-CSFs to (R288A)GR were greater than the corresponding ratios with WT-GR, suggesting a synergistic effect of receptor and G-CSF mutations.	bind
15616	1	5886	5	NULL	NULL	0	NULL	mAb 8E6	NULL		does not block	NULL	directly			PAI-1	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_11_9395_s_333	11773078	(Table  I), together with the observation that mAb 8E6 does not directly block PAI-1 binding (Figs.  6 and  7), argues that the observed inhibition reflects steric interference of PAI-1 binding to one site rather than the existence of two distinct PAI-1 binding sites.	bind
18121	1	5886	7	NULL	NULL	NULL	NULL	mAb 8E6	GP		does not block		directly			PAI-1	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_11_9395_s_333	11773078	(Table  I), together with the observation that mAb 8E6 does not directly block PAI-1 binding (Figs.  6 and  7), argues that the observed inhibition reflects steric interference of PAI-1 binding to one site rather than the existence of two distinct PAI-1 binding sites.	bind
15317	1	5888	5	10	NULL	0	NULL	isoproterenol 			increased		robustly			cAMP 		levels of			NULL	CHO cells expressing beta2-adrenergic receptor	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_8_5692_s_126	11069896	(Table  I), whereas isoproterenol (2 muM) caused a robust 6-fold increase in cAMP levels in CHO cells expressing the beta2-adrenergic receptor.	bind
18126	1	5888	7	NULL	NULL	NULL	NULL	isoproterenol	Chemical		increase		robustly			cAMP	Chemical	levels of			NULL	CHO cells expressing the beta2-adrenergic receptor	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_8_5692_s_126	11069896	(Table  I), whereas isoproterenol (2 muM) caused a robust 6-fold increase in cAMP levels in CHO cells expressing the beta2-adrenergic receptor.	bind
15318	1	5892	5	NULL	NULL	0	NULL	hdm2	NULL		bind	NULL				p53	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_17_2_554_s_264	9430646	(Table  I); both hdm2 and E1B-55 kDa proteins bind to p53 (Sarnow  et al., 1982  ; Momand  et al., 1992  ).	bind
15320	2	5892	5	NULL	NULL	0	NULL	E1B-55 kDa protein	NULL		bind	NULL				p53	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_17_2_554_s_264	9430646	(Table  I); both hdm2 and E1B-55 kDa proteins bind to p53 (Sarnow  et al., 1982  ; Momand  et al., 1992  ).	bind
18127	1	5892	7	NULL	NULL	NULL	NULL	hdm2	GP		bind					p53	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_2_554_s_264	9430646	(Table  I); both hdm2 and E1B-55 kDa proteins bind to p53 (Sarnow  et al., 1982  ; Momand  et al., 1992  ).	bind
18128	2	5892	7	NULL	NULL	NULL	NULL	E1B-55 kDa protein	GP		bind					p53	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_2_554_s_264	9430646	(Table  I); both hdm2 and E1B-55 kDa proteins bind to p53 (Sarnow  et al., 1982  ; Momand  et al., 1992  ).	bind
15354	1	5893	5	NULL	NULL	0	NULL	enzymes	NULL	mutant	bind	NULL	efficiently			tRNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_32_22225_s_179	10428788	(Table  I, Fig.  3) indicate that the mutant enzymes still bind tRNA efficiently, which argues against a large structural change.	bind
18130	1	5893	7	NULL	NULL	0	NULL	enzymes	NULL	mutant	bind	NULL	efficiently			tRNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_32_22225_s_179	10428788	(Table  I, Fig.  3) indicate that the mutant enzymes still bind tRNA efficiently, which argues against a large structural change.	bind
15355	1	5894	5	NULL	NULL	0	NULL	HIV-1 RT	NULL		bind	NULL				dNTPs	NULL	incorrect			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_25_22662_s_222	11927582	(Table  I; Ref.  15); however, the difference is that HIV-1 RT (micromolar  K d) binds incorrect dNTPs better than the T7 DNA polymerase (millimolar  K d; Ref.  30).	bind
15356	2	5894	5	NULL	NULL	0	NULL	HIV-1 RT	NULL		bind	NULL				T7 DNA polymerase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_25_22662_s_222	11927582	(Table  I; Ref.  15); however, the difference is that HIV-1 RT (micromolar  K d) binds incorrect dNTPs better than the T7 DNA polymerase (millimolar  K d; Ref.  30).	bind
15357	3	5894	5	NULL	NULL	0	NULL	statement 1	NULL		better than	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_25_22662_s_222	11927582	(Table  I; Ref.  15); however, the difference is that HIV-1 RT (micromolar  K d) binds incorrect dNTPs better than the T7 DNA polymerase (millimolar  K d; Ref.  30).	bind
18131	1	5894	7	NULL	NULL	NULL	NULL	HIV-1 RT	GP		binds					dNTPs	Chemical	incorrect			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_25_22662_s_222	11927582	(Table  I; Ref.  15); however, the difference is that HIV-1 RT (micromolar  K d) binds incorrect dNTPs better than the T7 DNA polymerase (millimolar  K d; Ref.  30).	bind
18132	2	5894	7	NULL	NULL	NULL	NULL	HIV-1 RT	GP		binds					T7 DNA polymerase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_25_22662_s_222	11927582	(Table  I; Ref.  15); however, the difference is that HIV-1 RT (micromolar  K d) binds incorrect dNTPs better than the T7 DNA polymerase (millimolar  K d; Ref.  30).	bind
18133	3	5894	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs better than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_25_22662_s_222	11927582	(Table  I; Ref.  15); however, the difference is that HIV-1 RT (micromolar  K d) binds incorrect dNTPs better than the T7 DNA polymerase (millimolar  K d; Ref.  30).	bind
15358	1	5895	5	NULL	NULL	0	NULL	CREB	NULL		bind	NULL					NULL			cAMP-response element	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_41_31708_s_161	10913126	(Table  I; TCG AGGTCA, TCA TGGCCA) ( 4) or the inhibin alpha gene, where SF-1 regulates gene transcription through its interaction with CREB bound to the cAMP-response element ( 17).	bind
15359	2	5895	5	NULL	NULL	0	NULL	SF-1	NULL		interacts with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_41_31708_s_161	10913126	(Table  I; TCG AGGTCA, TCA TGGCCA) ( 4) or the inhibin alpha gene, where SF-1 regulates gene transcription through its interaction with CREB bound to the cAMP-response element ( 17).	bind
15360	3	5895	5	NULL	NULL	0	NULL	SF-1	NULL		regulate	NULL				gene transcription	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_41_31708_s_161	10913126	(Table  I; TCG AGGTCA, TCA TGGCCA) ( 4) or the inhibin alpha gene, where SF-1 regulates gene transcription through its interaction with CREB bound to the cAMP-response element ( 17).	bind
15361	4	5895	5	NULL	NULL	0	NULL	statement 3	NULL		occurs through	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_41_31708_s_161	10913126	(Table  I; TCG AGGTCA, TCA TGGCCA) ( 4) or the inhibin alpha gene, where SF-1 regulates gene transcription through its interaction with CREB bound to the cAMP-response element ( 17).	bind
18136	1	5895	7	NULL	NULL	NULL	NULL	CREB	GP		bind									cAMP-response element	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_31708_s_161	10913126	(Table  I; TCG AGGTCA, TCA TGGCCA) ( 4) or the inhibin alpha gene, where SF-1 regulates gene transcription through its interaction with CREB bound to the cAMP-response element ( 17).	bind
18137	2	5895	7	NULL	NULL	NULL	NULL	SF-1	GP		regulates					gene transcription	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_31708_s_161	10913126	(Table  I; TCG AGGTCA, TCA TGGCCA) ( 4) or the inhibin alpha gene, where SF-1 regulates gene transcription through its interaction with CREB bound to the cAMP-response element ( 17).	bind
18139	3	5895	7	NULL	NULL	NULL	NULL	statement 2	Process		occurs through					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_31708_s_161	10913126	(Table  I; TCG AGGTCA, TCA TGGCCA) ( 4) or the inhibin alpha gene, where SF-1 regulates gene transcription through its interaction with CREB bound to the cAMP-response element ( 17).	bind
15362	1	5896	5	NULL	NULL	0	NULL	POPC-apoE4	NULL		bind	NULL				ldlA cells	NULL		Q402R/Q418		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_24_21149_s_237	11861652	(Table  II) as well as with the reduced binding of POPC-apoE4 to the ldlA [Q402R/Q418] cells (Fig.  3 D) ( 28).	bind
18140	1	5896	7	NULL	NULL	NULL	NULL	POPC-apoE4 	GP		bind					 ldlA cells	Cell		Q402R/Q418		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_24_21149_s_237	11861652	(Table  II) as well as with the reduced binding of POPC-apoE4 to the ldlA [Q402R/Q418] cells (Fig.  3 D) ( 28).	bind
15363	1	5897	5	NULL	NULL	0	NULL	htf	NULL		bind	NULL				TbpB	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_17_14712_s_140	12571247	(Table  II) in all of the experiments was found to be close to 1, confirming the previously suggested 1:1 stoichiometry for the binding of htf to TbpB ( ).	bind
18144	1	5897	7	NULL	NULL	NULL	NULL	htf 	GP		bind					TbpB	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_17_14712_s_140	12571247	(Table  II) in all of the experiments was found to be close to 1, confirming the previously suggested 1:1 stoichiometry for the binding of htf to TbpB ( ).	bind
15364	1	5899	5	NULL	NULL	0	NULL	sCPS	NULL		bind	NULL				UMP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_47_45466_s_203	12244118	(Table  II) that sCPS bound both UMP and IMP and that chCPS bound IMP were unexpected because none of these interactions had been revealed by effects on enzymatic activity.	bind
15365	2	5899	5	NULL	NULL	0	NULL	sCPS	NULL		bind	NULL				IMP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_47_45466_s_203	12244118	(Table  II) that sCPS bound both UMP and IMP and that chCPS bound IMP were unexpected because none of these interactions had been revealed by effects on enzymatic activity.	bind
15366	3	5899	5	NULL	NULL	0	NULL	chCPS	NULL		bind	NULL				IMP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_47_45466_s_203	12244118	(Table  II) that sCPS bound both UMP and IMP and that chCPS bound IMP were unexpected because none of these interactions had been revealed by effects on enzymatic activity.	bind
18145	2	5899	7	NULL	NULL	NULL	NULL	sCPS	GP		bind					 IMP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_47_45466_s_203	12244118	(Table  II) that sCPS bound both UMP and IMP and that chCPS bound IMP were unexpected because none of these interactions had been revealed by effects on enzymatic activity.	bind
18147	1	5899	7	NULL	NULL	NULL	NULL	sCPS	GP		bind					 UMP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_47_45466_s_203	12244118	(Table  II) that sCPS bound both UMP and IMP and that chCPS bound IMP were unexpected because none of these interactions had been revealed by effects on enzymatic activity.	bind
18148	3	5899	7	NULL	NULL	NULL	NULL	chCPS	GP		bind					IMP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_47_45466_s_203	12244118	(Table  II) that sCPS bound both UMP and IMP and that chCPS bound IMP were unexpected because none of these interactions had been revealed by effects on enzymatic activity.	bind
15367	1	5900	5	NULL	NULL	0	NULL	factor VIIa	NULL	helix residues	bind	NULL				TF	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_26_18477_s_351	10373456	(Table  II) that the corresponding helix residues in factor VIIa bind to TF ( 4) and in factor Xa, they are involved in binding to factor Va. 4 Thus, a common function of this helix (162 in chymotrypsin numbering) in several blood coagulation proteases may be to serve as a binding site for the respective cofactor.	bind
15368	2	5900	5	NULL	NULL	0	NULL	factor Xa	NULL	helix residues	bind	NULL				factor Va	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_26_18477_s_351	10373456	(Table  II) that the corresponding helix residues in factor VIIa bind to TF ( 4) and in factor Xa, they are involved in binding to factor Va. 4 Thus, a common function of this helix (162 in chymotrypsin numbering) in several blood coagulation proteases may be to serve as a binding site for the respective cofactor.	bind
54129	3	5900	5	10	NULL	0	NULL	chymotrypsin			serve as		may	helix 162		cofactor			binding site		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_26_18477_s_351	10373456	(Table  II) that the corresponding helix residues in factor VIIa bind to TF ( 4) and in factor Xa, they are involved in binding to factor Va. 4 Thus, a common function of this helix (162 in chymotrypsin numbering) in several blood coagulation proteases may be to serve as a binding site for the respective cofactor.	bind
18150	1	5900	7	NULL	NULL	NULL	NULL	factor VIIa	GP		bind			helix residues		TF	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_26_18477_s_351	10373456	(Table  II) that the corresponding helix residues in factor VIIa bind to TF ( 4) and in factor Xa, they are involved in binding to factor Va. 4 Thus, a common function of this helix (162 in chymotrypsin numbering) in several blood coagulation proteases may be to serve as a binding site for the respective cofactor.	bind
18151	2	5900	7	NULL	NULL	NULL	NULL	factor Xa	GP		bind			helix residues		 factor Va	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_26_18477_s_351	10373456	(Table  II) that the corresponding helix residues in factor VIIa bind to TF ( 4) and in factor Xa, they are involved in binding to factor Va. 4 Thus, a common function of this helix (162 in chymotrypsin numbering) in several blood coagulation proteases may be to serve as a binding site for the respective cofactor.	bind
18157	3	5900	7	NULL	NULL	NULL	NULL	chymotrypsin	GP		serve as			helix 162		cofactor	GP	binding site for			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_26_18477_s_351	10373456	(Table  II) that the corresponding helix residues in factor VIIa bind to TF ( 4) and in factor Xa, they are involved in binding to factor Va. 4 Thus, a common function of this helix (162 in chymotrypsin numbering) in several blood coagulation proteases may be to serve as a binding site for the respective cofactor.	bind
15369	1	5901	5	NULL	NULL	0	NULL	gp120	NULL		bind	NULL				V3-BPs	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_34_21988_s_278	9705340	(Table  II), and that the pseudopeptide inhibitor of HIV entry that mimics the V3 loop blocks the binding of gp120 to the V3-BPs (Fig.  6 B).	bind
15370	2	5901	5	NULL	NULL	0	NULL	pseudopeptide inhibitor of HIV	NULL		mimics	NULL				V3 loop	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_34_21988_s_278	9705340	(Table  II), and that the pseudopeptide inhibitor of HIV entry that mimics the V3 loop blocks the binding of gp120 to the V3-BPs (Fig.  6 B).	bind
15371	3	5901	5	NULL	NULL	0	NULL	statement 2	NULL		blocks	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_34_21988_s_278	9705340	(Table  II), and that the pseudopeptide inhibitor of HIV entry that mimics the V3 loop blocks the binding of gp120 to the V3-BPs (Fig.  6 B).	bind
18159	1	5901	7	NULL	NULL	NULL	NULL	gp120	GP		bind					V3-BPs	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_34_21988_s_278	9705340	(Table  II), and that the pseudopeptide inhibitor of HIV entry that mimics the V3 loop blocks the binding of gp120 to the V3-BPs (Fig.  6 B).	bind
18160	2	5901	7	NULL	NULL	NULL	NULL	pseudopeptide inhibitor of HIV	GP		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_34_21988_s_278	9705340	(Table  II), and that the pseudopeptide inhibitor of HIV entry that mimics the V3 loop blocks the binding of gp120 to the V3-BPs (Fig.  6 B).	bind
18161	3	5901	7	NULL	NULL	NULL	NULL	pseudopeptide inhibitor of HIV	GP		mimics					V3 loop	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_34_21988_s_278	9705340	(Table  II), and that the pseudopeptide inhibitor of HIV entry that mimics the V3 loop blocks the binding of gp120 to the V3-BPs (Fig.  6 B).	bind
15372	1	5904	5	NULL	NULL	0	NULL	P450c27	NULL		bind	NULL				Adx	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_4_2045_s_112	9890963	(Table  II), confirming the original chromatographic observation that P450c27 binds much more tightly to Adx than P450scc.	bind
15373	2	5904	5	NULL	NULL	0	NULL	P450c27	NULL		bind	NULL				P450scc	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_4_2045_s_112	9890963	(Table  II), confirming the original chromatographic observation that P450c27 binds much more tightly to Adx than P450scc.	bind
20338	3	5904	5	NULL	NULL	0	NULL	statement 1	NULL	affinity of	is greater than	NULL				statement 2	NULL	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_4_2045_s_112	9890963	(Table  II), confirming the original chromatographic observation that P450c27 binds much more tightly to Adx than P450scc.	bind
18218	1	5904	7	NULL	NULL	NULL	NULL	P450c27 	GP		binds					Adx 	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_4_2045_s_112	9890963	(Table  II), confirming the original chromatographic observation that P450c27 binds much more tightly to Adx than P450scc.	bind
18219	2	5904	7	NULL	NULL	NULL	NULL	P450scc	GP		binds					Adx	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_4_2045_s_112	9890963	(Table  II), confirming the original chromatographic observation that P450c27 binds much more tightly to Adx than P450scc.	bind
18220	3	5904	7	NULL	NULL	NULL	NULL	statement 1	Process	affinity of	is greater than					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_4_2045_s_112	9890963	(Table  II), confirming the original chromatographic observation that P450c27 binds much more tightly to Adx than P450scc.	bind
15374	1	5906	5	NULL	NULL	0	NULL	ATP	NULL		bind	NULL	allosteric				NULL		Fru-2,6-P2ase domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_27_24608_s_114	11325970	(Table  II), it is likely that the ATP activation of the chicken liver 6PF-2K is caused by allosteric binding of ATP to the Fru-2,6-P2ase domain.	bind
15375	2	5906	5	10	NULL	0	NULL	ATP			activates					6PF-2K		chicken;;liver			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_24608_s_114	11325970	(Table  II), it is likely that the ATP activation of the chicken liver 6PF-2K is caused by allosteric binding of ATP to the Fru-2,6-P2ase domain.	bind
20339	3	5906	5	NULL	NULL	0	NULL	statement 1	NULL		causes	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_27_24608_s_114	11325970	(Table  II), it is likely that the ATP activation of the chicken liver 6PF-2K is caused by allosteric binding of ATP to the Fru-2,6-P2ase domain.	bind
18221	1	5906	7	NULL	NULL	NULL	NULL	ATP	Chemical		binds		allosterically						Fru-2,6-P2ase domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_24608_s_114	11325970	(Table  II), it is likely that the ATP activation of the chicken liver 6PF-2K is caused by allosteric binding of ATP to the Fru-2,6-P2ase domain.	bind
18222	2	5906	7	NULL	NULL	NULL	NULL	ATP	Chemical		activates					6PF-2K 	GP	chicken;;liver			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_24608_s_114	11325970	(Table  II), it is likely that the ATP activation of the chicken liver 6PF-2K is caused by allosteric binding of ATP to the Fru-2,6-P2ase domain.	bind
18223	3	5906	7	NULL	NULL	NULL	NULL	statement 1	Process		cause					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_24608_s_114	11325970	(Table  II), it is likely that the ATP activation of the chicken liver 6PF-2K is caused by allosteric binding of ATP to the Fru-2,6-P2ase domain.	bind
15376	1	5907	5	10	NULL	0	NULL	aptamer DP3	NULL		mimics	NULL	closely			Y2 receptor	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_13_11416_s_242	11756401	(Table  II), strongly suggest that the aptamer DP3 mimics the binding behavior of the Y2 receptor more closely than that of the Y1 and Y5 receptors.	bind
15377	2	5907	5	10	NULL	0	NULL	aptamer DP3	NULL		mimics	NULL				Y1 receptor	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_13_11416_s_242	11756401	(Table  II), strongly suggest that the aptamer DP3 mimics the binding behavior of the Y2 receptor more closely than that of the Y1 and Y5 receptors.	bind
15378	3	5907	5	10	NULL	0	NULL	aptamer DP3	NULL		mimics	NULL				Y5 receptor	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_13_11416_s_242	11756401	(Table  II), strongly suggest that the aptamer DP3 mimics the binding behavior of the Y2 receptor more closely than that of the Y1 and Y5 receptors.	bind
20340	4	5907	5	NULL	NULL	0	NULL	statement 1	NULL		 is more close than	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_13_11416_s_242	11756401	(Table  II), strongly suggest that the aptamer DP3 mimics the binding behavior of the Y2 receptor more closely than that of the Y1 and Y5 receptors.	bind
20341	5	5907	5	NULL	NULL	0	NULL	statement 1	NULL		 is more close than	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_13_11416_s_242	11756401	(Table  II), strongly suggest that the aptamer DP3 mimics the binding behavior of the Y2 receptor more closely than that of the Y1 and Y5 receptors.	bind
18224	1	5907	7	NULL	NULL	NULL	NULL	aptamer DP3	GP		mimics					Y2 receptor	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_13_11416_s_242	11756401	(Table  II), strongly suggest that the aptamer DP3 mimics the binding behavior of the Y2 receptor more closely than that of the Y1 and Y5 receptors.	bind
18225	2	5907	7	NULL	NULL	NULL	NULL	aptamer DP3	GP		mimics					Y1 receptor	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_13_11416_s_242	11756401	(Table  II), strongly suggest that the aptamer DP3 mimics the binding behavior of the Y2 receptor more closely than that of the Y1 and Y5 receptors.	bind
18226	3	5907	7	NULL	NULL	NULL	NULL	aptamer DP3	GP		mimics					Y5 receptor	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_13_11416_s_242	11756401	(Table  II), strongly suggest that the aptamer DP3 mimics the binding behavior of the Y2 receptor more closely than that of the Y1 and Y5 receptors.	bind
18227	4	5907	7	NULL	NULL	NULL	NULL	statement 1	Process		is more close than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_13_11416_s_242	11756401	(Table  II), strongly suggest that the aptamer DP3 mimics the binding behavior of the Y2 receptor more closely than that of the Y1 and Y5 receptors.	bind
18228	5	5907	7	NULL	NULL	NULL	NULL	statement 1	Process		is more close than					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_13_11416_s_242	11756401	(Table  II), strongly suggest that the aptamer DP3 mimics the binding behavior of the Y2 receptor more closely than that of the Y1 and Y5 receptors.	bind
15379	1	5908	5	NULL	NULL	0	NULL	Cl	NULL		bind	NULL	only			EA state	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_4_2232_s_154	9442066	(Table  II), strongly suggesting that Cl  binds only to the  EA state.	bind
18229	1	5908	7	NULL	NULL	NULL	NULL	Cl	Chemical		binds		only			EA state	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_4_2232_s_154	9442066	(Table  II), strongly suggesting that Cl  binds only to the  EA state.	bind
15380	1	5910	5	NULL	NULL	0	NULL	eIF4E	NULL		bind	NULL				eIF4G1-459	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_29_21817_s_345	10764794	(Table  II), we tested the hypothesis that excess Rbp29p may increase the binding of eIF4E to eIF4G1-459.	bind
20342	2	5910	5	NULL	NULL	0	NULL	Rbp29p	NULL		increase	NULL	may			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_29_21817_s_345	10764794	(Table  II), we tested the hypothesis that excess Rbp29p may increase the binding of eIF4E to eIF4G1-459.	bind
18230	1	5910	7	NULL	NULL	NULL	NULL	eIF4E	GP		bind					eIF4G	GP		1-459		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_29_21817_s_345	10764794	(Table  II), we tested the hypothesis that excess Rbp29p may increase the binding of eIF4E to eIF4G1-459.	bind
18231	2	5910	7	NULL	NULL	NULL	NULL	Rbp29p	GP	excess of	increase		may			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_29_21817_s_345	10764794	(Table  II), we tested the hypothesis that excess Rbp29p may increase the binding of eIF4E to eIF4G1-459.	bind
15381	2	5911	5	10	NULL	0	NULL	statement 1			does not bind					protein S					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_15144_s_206	10329721	(Table  II), whereas constructs lacking SCR-1 did not bind to protein S (Figs.  3 and  4).	bind
54134	1	5911	5	10	NULL	0	NULL	constructs			lacks					SCR-1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_21_15144_s_206	10329721	(Table  II), whereas constructs lacking SCR-1 did not bind to protein S (Figs.  3 and  4).	bind
18232	2	5911	7	NULL	NULL	NULL	NULL	statement 1	Process		does not bind					protein S	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_15144_s_206	10329721	(Table  II), whereas constructs lacking SCR-1 did not bind to protein S (Figs.  3 and  4).	bind
54136	1	5911	7	NULL	NULL	NULL	NULL	constructs	GP		lacks					SCR-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_15144_s_206	10329721	(Table  II), whereas constructs lacking SCR-1 did not bind to protein S (Figs.  3 and  4).	bind
15382	1	5913	5	NULL	NULL	0	NULL	NT-3	NULL		bind	NULL				CR1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_11_7870_s_166	10713102	(Table  III), in agreement with NT-3 binding better to CR1 than to CR13	bind
15383	2	5913	5	NULL	NULL	0	NULL	NT-3	NULL		bind	NULL				CR13	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_11_7870_s_166	10713102	(Table  III), in agreement with NT-3 binding better to CR1 than to CR13	bind
15384	3	5913	5	NULL	NULL	0	NULL	statement 1	NULL		better than	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_11_7870_s_166	10713102	(Table  III), in agreement with NT-3 binding better to CR1 than to CR13	bind
18233	1	5913	7	NULL	NULL	NULL	NULL	NT-3	GP		bind					CR1 	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_11_7870_s_166	10713102	(Table  III), in agreement with NT-3 binding better to CR1 than to CR13	bind
18234	2	5913	7	NULL	NULL	NULL	NULL	NT-3	GP		bind					CR13	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_11_7870_s_166	10713102	(Table  III), in agreement with NT-3 binding better to CR1 than to CR13	bind
18235	3	5913	7	NULL	NULL	NULL	NULL	statement 1	Process		is better than 					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_11_7870_s_166	10713102	(Table  III), in agreement with NT-3 binding better to CR1 than to CR13	bind
15385	1	5914	5	NULL	NULL	0	NULL	pGH	NULL		bind	NULL	poorly			GH receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_43_27077_s_164	9341147	(Table  III), so the residual 17-fold loss in affinity may be a result of generally poorer binding of pGH to GH receptors.	bind
18236	1	5914	7	NULL	NULL	NULL	NULL	pGH	GP		binds		poorly			GH receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_43_27077_s_164	9341147	(Table  III), so the residual 17-fold loss in affinity may be a result of generally poorer binding of pGH to GH receptors.	bind
15386	1	5915	5	NULL	NULL	0	NULL	CD62L	NULL		bind	NULL				GlyCAM-1 	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_2_763_s_201	9422729	(Table  III), two major capping groups present in GlyCAM-1  O-linked oligosaccharides ( 53,  54), are only slightly higher (250-800 muM) than the  K d measured in the present study for CD62L binding to GlyCAM-1 (~108 muM).	bind
18237	1	5915	7	NULL	NULL	NULL	NULL	CD62L 	GP		binds					GlyCAM-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_2_763_s_201	9422729	(Table  III), two major capping groups present in GlyCAM-1  O-linked oligosaccharides ( 53,  54), are only slightly higher (250-800 muM) than the  K d measured in the present study for CD62L binding to GlyCAM-1 (~108 muM).	bind
15387	1	5918	5	10	NULL	0	NULL	mAb 2C7 	NULL		bind	NULL				WG LOS	NULL	inner structure of	15253 LOS		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_51_36550_s_186	10593954	(Table  IV), which confirmed that mAb 2C7 bound to the inner 15253 LOS structure within WG LOS.	bind
18238	1	5918	7	NULL	NULL	NULL	NULL	mAb 2C7	GP		bind					WG LOS	GP	inner structure of	15253 LOS 		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_51_36550_s_186	10593954	(Table  IV), which confirmed that mAb 2C7 bound to the inner 15253 LOS structure within WG LOS.	bind
15389	1	5919	5	NULL	NULL	0	NULL	htf	NULL		bind	NULL				His6-TbpB	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_17_14712_s_246	12571247	(Table  VI) for htf binding to N-ter was about three times largerR than the corresponding value for the binding to His6-TbpB.	bind
18239	1	5919	7	NULL	NULL	NULL	NULL	htf	GP		bind					His6-TbpB	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_17_14712_s_246	12571247	(Table  VI) for htf binding to N-ter was about three times largerR than the corresponding value for the binding to His6-TbpB.	bind
15391	1	5920	5	NULL	NULL	0	NULL	A26	NULL		bind	NULL				TeR-2 DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_25_15881_s_287	9188487	(Table  VI), A26 binds TeR-2 DNA less tightly than TeR-4 DNA ( 71).	bind
15392	2	5920	5	NULL	NULL	0	NULL	A26	NULL		bind	NULL				TeR-4 DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_25_15881_s_287	9188487	(Table  VI), A26 binds TeR-2 DNA less tightly than TeR-4 DNA ( 71).	bind
15393	3	5920	5	NULL	NULL	0	NULL	statement 1	NULL		less tightly than	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_25_15881_s_287	9188487	(Table  VI), A26 binds TeR-2 DNA less tightly than TeR-4 DNA ( 71).	bind
18240	1	5920	7	NULL	NULL	NULL	NULL	A26	GP		binds					TeR-2 DNA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_25_15881_s_287	9188487	(Table  VI), A26 binds TeR-2 DNA less tightly than TeR-4 DNA ( 71).	bind
18241	2	5920	7	NULL	NULL	NULL	NULL	A26	GP		binds					TeR-4 DNA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_25_15881_s_287	9188487	(Table  VI), A26 binds TeR-2 DNA less tightly than TeR-4 DNA ( 71).	bind
18242	3	5920	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs less tightly than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_25_15881_s_287	9188487	(Table  VI), A26 binds TeR-2 DNA less tightly than TeR-4 DNA ( 71).	bind
15395	1	5921	5	NULL	NULL	0	NULL	repressor	NULL	putative	bind	NULL					NULL			RE3	NULL		NULL	NULL	NULL	NULL	gw60_embo_16_10_2554_s_191	9184203	(Table  VI), indicating that the putative repressor that binds to RE3 requires both signalling molecules for activation.	bind
15396	2	5921	5	10	NULL	0	NULL	repressor		activation of;;putative	requires					signalling molecules					NULL		NULL	NULL	NULL	NULL	gw60_embo_16_10_2554_s_191	9184203	(Table  VI), indicating that the putative repressor that binds to RE3 requires both signalling molecules for activation.	bind
18243	1	5921	7	NULL	NULL	NULL	NULL			putative	binds to				 repressor					RE3	NULL		NULL	NULL	NULL	NULL	gw60_embo_16_10_2554_s_191	9184203	(Table  VI), indicating that the putative repressor that binds to RE3 requires both signalling molecules for activation.	bind
18244	2	5921	7	NULL	NULL	NULL	NULL	repressor	GP	activation of;;putative	requires					signalling molecules	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_10_2554_s_191	9184203	(Table  VI), indicating that the putative repressor that binds to RE3 requires both signalling molecules for activation.	bind
15397	1	5923	5	NULL	NULL	0	NULL	CRP	NULL	purified	bind	NULL				cai-fix	NULL			intergenic promoter region	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbacteriol_180_10_2599_s_235	9573142	(Tables  2 and  3), the binding specificity of purified CRP to the  cai-fix intergenic promoter region was tested in vitro by performing gel mobility shift assays.	bind
18245	1	5923	7	NULL	NULL	NULL	NULL	CRP	GP	purified	binds					cai-fix	GP			 intergenic promoter	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbacteriol_180_10_2599_s_235	9573142	(Tables  2 and  3), the binding specificity of purified CRP to the  cai-fix intergenic promoter region was tested in vitro by performing gel mobility shift assays.	bind
15398	1	5924	5	NULL	NULL	0	NULL	Pot1N molecule	NULL	additional	bind	NULL				(Tel)4	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_9119_s_176	15637058	(TelAC)3 complex (compare  lanes 2 and  3), suggesting that an additional Pot1N molecule was bound to (Tel)4.	bind
18246	1	5924	7	NULL	NULL	NULL	NULL	Pot1N molecule	GP		bind					(Tel)4	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_10_9119_s_176	15637058	(TelAC)3 complex (compare  lanes 2 and  3), suggesting that an additional Pot1N molecule was bound to (Tel)4.	bind
15399	1	5925	5	NULL	NULL	0	NULL	FVIIa	NULL		bind	NULL				TF	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_49_45895_s_58	11590156	(TF9 10H10 antibody binds to TF without interfering FVIIa binding to TF.)	bind
15400	2	5925	5	NULL	NULL	0	NULL	TF9 10H10 antibody	NULL		bind	NULL				TF	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_49_45895_s_58	11590156	(TF9 10H10 antibody binds to TF without interfering FVIIa binding to TF.)	bind
15401	3	5925	5	10	NULL	0	NULL	statement 2			does not interfere with					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_49_45895_s_58	11590156	(TF9 10H10 antibody binds to TF without interfering FVIIa binding to TF.)	bind
18247	1	5925	7	NULL	NULL	NULL	NULL	TF9 10H10 antibody	GP		binds to					TF	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_49_45895_s_58	11590156	(TF9 10H10 antibody binds to TF without interfering FVIIa binding to TF.)	bind
18248	2	5925	7	NULL	NULL	NULL	NULL	FVIIa	GP		binds to					TF	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_49_45895_s_58	11590156	(TF9 10H10 antibody binds to TF without interfering FVIIa binding to TF.)	bind
18249	3	5925	7	NULL	NULL	NULL	NULL	statement 1	Process		does not interfere with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_49_45895_s_58	11590156	(TF9 10H10 antibody binds to TF without interfering FVIIa binding to TF.)	bind
15402	1	5926	5	NULL	NULL	0	NULL	TGFbeta-receptor-associated protein	NULL		interacts with	NULL				receptor complex	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_23_2783_s_161	16322555	(TGFbeta-receptor-associated protein) (Wurthner et al. 2001 ) and TLP (TRAP-1-like protein) (Felici et al. 2003 ) have been described as adaptor proteins that interact with the receptor complex and facilitate the formation of Smad2/3 - Smad4 complexes.	bind
15403	2	5926	5	NULL	NULL	0	NULL	TGFbeta-receptor-associated protein	NULL		facilitate	NULL				Smad2/3 - Smad4 complexes	NULL	formation of			NULL		0	NULL	NULL	NULL	gw70_genesdev_19_23_2783_s_161	16322555	(TGFbeta-receptor-associated protein) (Wurthner et al. 2001 ) and TLP (TRAP-1-like protein) (Felici et al. 2003 ) have been described as adaptor proteins that interact with the receptor complex and facilitate the formation of Smad2/3 - Smad4 complexes.	bind
15404	3	5926	5	NULL	NULL	0	NULL	TLP	NULL		is	NULL				TRAP-1-like protein	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_23_2783_s_161	16322555	(TGFbeta-receptor-associated protein) (Wurthner et al. 2001 ) and TLP (TRAP-1-like protein) (Felici et al. 2003 ) have been described as adaptor proteins that interact with the receptor complex and facilitate the formation of Smad2/3 - Smad4 complexes.	bind
15405	4	5926	5	NULL	NULL	0	NULL	TLP	NULL		interacts with	NULL				receptor complex	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_23_2783_s_161	16322555	(TGFbeta-receptor-associated protein) (Wurthner et al. 2001 ) and TLP (TRAP-1-like protein) (Felici et al. 2003 ) have been described as adaptor proteins that interact with the receptor complex and facilitate the formation of Smad2/3 - Smad4 complexes.	bind
15406	5	5926	5	NULL	NULL	0	NULL	TLP	NULL		facilitate	NULL				Smad2/3 - Smad4 complexes	NULL	formation of			NULL		0	NULL	NULL	NULL	gw70_genesdev_19_23_2783_s_161	16322555	(TGFbeta-receptor-associated protein) (Wurthner et al. 2001 ) and TLP (TRAP-1-like protein) (Felici et al. 2003 ) have been described as adaptor proteins that interact with the receptor complex and facilitate the formation of Smad2/3 - Smad4 complexes.	bind
44840	6	5926	5	NULL	NULL	0	NULL	TGFbeta-receptor-associated protein	NULL		is a type of	NULL				adaptor protein	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_23_2783_s_161	16322555	(TGFbeta-receptor-associated protein) (Wurthner et al. 2001 ) and TLP (TRAP-1-like protein) (Felici et al. 2003 ) have been described as adaptor proteins that interact with the receptor complex and facilitate the formation of Smad2/3 - Smad4 complexes.	bind
44841	7	5926	5	NULL	NULL	0	NULL	TLP	NULL		is a type of	NULL				adaptor protein	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_23_2783_s_161	16322555	(TGFbeta-receptor-associated protein) (Wurthner et al. 2001 ) and TLP (TRAP-1-like protein) (Felici et al. 2003 ) have been described as adaptor proteins that interact with the receptor complex and facilitate the formation of Smad2/3 - Smad4 complexes.	bind
18250	1	5926	7	NULL	NULL	NULL	NULL	TGFbeta-receptor-associated protein	GP		interact with					receptor complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_23_2783_s_161	16322555	(TGFbeta-receptor-associated protein) (Wurthner et al. 2001 ) and TLP (TRAP-1-like protein) (Felici et al. 2003 ) have been described as adaptor proteins that interact with the receptor complex and facilitate the formation of Smad2/3 - Smad4 complexes.	bind
18251	2	5926	7	NULL	NULL	NULL	NULL	TLP	GP		interacts with					receptor complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_23_2783_s_161	16322555	(TGFbeta-receptor-associated protein) (Wurthner et al. 2001 ) and TLP (TRAP-1-like protein) (Felici et al. 2003 ) have been described as adaptor proteins that interact with the receptor complex and facilitate the formation of Smad2/3 - Smad4 complexes.	bind
18252	3	5926	7	NULL	NULL	NULL	NULL	statement 1	Process		facilitate					Smad2/3 - Smad4 complexes	GP	formation of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_23_2783_s_161	16322555	(TGFbeta-receptor-associated protein) (Wurthner et al. 2001 ) and TLP (TRAP-1-like protein) (Felici et al. 2003 ) have been described as adaptor proteins that interact with the receptor complex and facilitate the formation of Smad2/3 - Smad4 complexes.	bind
18253	7	5926	7	NULL	NULL	NULL	NULL	TLP	GP		is					TRAP-1-like protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_23_2783_s_161	16322555	(TGFbeta-receptor-associated protein) (Wurthner et al. 2001 ) and TLP (TRAP-1-like protein) (Felici et al. 2003 ) have been described as adaptor proteins that interact with the receptor complex and facilitate the formation of Smad2/3 - Smad4 complexes.	bind
18254	5	5926	7	NULL	NULL	NULL	NULL	TGFbeta-receptor-associated protein	GP		is a type of					adaptor protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_23_2783_s_161	16322555	(TGFbeta-receptor-associated protein) (Wurthner et al. 2001 ) and TLP (TRAP-1-like protein) (Felici et al. 2003 ) have been described as adaptor proteins that interact with the receptor complex and facilitate the formation of Smad2/3 - Smad4 complexes.	bind
18255	6	5926	7	NULL	NULL	NULL	NULL	TLP	GP		is a type of					adaptor protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_23_2783_s_161	16322555	(TGFbeta-receptor-associated protein) (Wurthner et al. 2001 ) and TLP (TRAP-1-like protein) (Felici et al. 2003 ) have been described as adaptor proteins that interact with the receptor complex and facilitate the formation of Smad2/3 - Smad4 complexes.	bind
45562	4	5926	7	NULL	NULL	NULL	NULL	statement 2	Process		facilitate					Smad2/3 - Smad4 complexes	GP	formation of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_23_2783_s_161	16322555	(TGFbeta-receptor-associated protein) (Wurthner et al. 2001 ) and TLP (TRAP-1-like protein) (Felici et al. 2003 ) have been described as adaptor proteins that interact with the receptor complex and facilitate the formation of Smad2/3 - Smad4 complexes.	bind
15407	1	5927	5	NULL	NULL	0	NULL	troponin	NULL	truncated	bind	NULL				tropomyosin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_43_25455_s_145	7592713	(The   Fig. 3results can only  be analyzed qualitatively because of uncertainty in the stoichiometry  of truncated troponin binding to tropomyosin and to the thin filament.)	bind
15408	2	5927	5	NULL	NULL	0	NULL	troponin	NULL	truncated	bind	NULL				thin filament	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_43_25455_s_145	7592713	(The   Fig. 3results can only  be analyzed qualitatively because of uncertainty in the stoichiometry  of truncated troponin binding to tropomyosin and to the thin filament.)	bind
18256	1	5927	7	NULL	NULL	NULL	NULL	troponin	GP	truncated	binds					tropomyosin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_43_25455_s_145	7592713	(The   Fig. 3results can only  be analyzed qualitatively because of uncertainty in the stoichiometry  of truncated troponin binding to tropomyosin and to the thin filament.)	bind
18257	2	5927	7	NULL	NULL	NULL	NULL	troponin	GP	truncated	binds to					thin filament	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_43_25455_s_145	7592713	(The   Fig. 3results can only  be analyzed qualitatively because of uncertainty in the stoichiometry  of truncated troponin binding to tropomyosin and to the thin filament.)	bind
15409	1	5930	5	NULL	NULL	0	NULL	4E-BP1	NULL		bind	NULL				eIF4E	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_16_9373_s_119	9545260	(The exception here (as in CHO cells) is arsenite, which does not cause increased binding of 4E-BP1 to eIF4E.	bind
15410	2	5930	5	10	NULL	0	NULL	arsenite	NULL		does not increase	NULL				statement 1	NULL	binding affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_16_9373_s_119	9545260	(The exception here (as in CHO cells) is arsenite, which does not cause increased binding of 4E-BP1 to eIF4E.	bind
18264	1	5930	7	NULL	NULL	NULL	NULL	4E-BP1	GP		bind					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_16_9373_s_119	9545260	(The exception here (as in CHO cells) is arsenite, which does not cause increased binding of 4E-BP1 to eIF4E.	bind
18265	2	5930	7	NULL	NULL	NULL	NULL	arsenite	Chemical		does not increase					statement 1	Process	binding affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_16_9373_s_119	9545260	(The exception here (as in CHO cells) is arsenite, which does not cause increased binding of 4E-BP1 to eIF4E.	bind
15411	1	5931	5	NULL	NULL	0	NULL	Ste7	NULL		bind	NULL				GST-Ste5 	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_20_9221_s_348	15456892	(The exception was for comparisons of Ste7 binding to GST-Ste5 [see below].)	bind
18266	1	5931	7	NULL	NULL	NULL	NULL	Ste7	GP		bind					GST-Ste5	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_9221_s_348	15456892	(The exception was for comparisons of Ste7 binding to GST-Ste5 [see below].)	bind
15412	1	5932	5	10	NULL	0	NULL	ALEX	NULL		bind	NULL	weakly			GST	NULL	alone			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_14_3849_s_193	11447126	(The low level binding of ALEX to GST alone presumably reflects an unspecific sticking of the highly basic ALEX.)	bind
18267	1	5932	7	NULL	NULL	NULL	NULL	ALEX	GP		binds		weakly			GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_14_3849_s_193	11447126	(The low level binding of ALEX to GST alone presumably reflects an unspecific sticking of the highly basic ALEX.)	bind
15413	1	5933	5	NULL	NULL	0	NULL	LacR	NULL		bind	NULL					NULL			operon O1	NULL		0	NULL	NULL	NULL	gw70_pnas_103_26_9879_s_65	16785444	(The probability of occurrence of a loop depends on the energies,  GO1 and  GO3, of LacR binding to operons O1 and O3, and the difference, delta G, between  GDNA and the free energy of an unbound DNA segment of identical length.)	bind
15414	2	5933	5	NULL	NULL	0	NULL	LacR	NULL		bind	NULL					NULL			operon O3	NULL		0	NULL	NULL	NULL	gw70_pnas_103_26_9879_s_65	16785444	(The probability of occurrence of a loop depends on the energies,  GO1 and  GO3, of LacR binding to operons O1 and O3, and the difference, delta G, between  GDNA and the free energy of an unbound DNA segment of identical length.)	bind
18271	1	5933	7	NULL	NULL	NULL	NULL	LacR	GP		bind									operon O1	NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_26_9879_s_65	16785444	(The probability of occurrence of a loop depends on the energies,  GO1 and  GO3, of LacR binding to operons O1 and O3, and the difference, delta G, between  GDNA and the free energy of an unbound DNA segment of identical length.)	bind
18272	2	5933	7	NULL	NULL	NULL	NULL	LacR	GP		bind									operon O3	NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_26_9879_s_65	16785444	(The probability of occurrence of a loop depends on the energies,  GO1 and  GO3, of LacR binding to operons O1 and O3, and the difference, delta G, between  GDNA and the free energy of an unbound DNA segment of identical length.)	bind
15417	1	5934	5	NULL	NULL	0	NULL	dyn-2	NULL		mediate	NULL		PRD		eNOS activity	NULL	potentiation of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_8_5894_s_13	12488320	(These data indicate that the binding domains of dyn-2 and eNOS reside within the dyn-2 PRD domain and the FAD binding region of the eNOS reductase domains, respectively, and that dyn-2 PRD is sufficient to mediate dyn-2-dependent potentiation of eNOS activity, at least in part, by potentiating electron transfer.)	bind
15418	2	5934	5	NULL	NULL	0	NULL	statement 1	NULL		dependent on	NULL				dyn-2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_8_5894_s_13	12488320	(These data indicate that the binding domains of dyn-2 and eNOS reside within the dyn-2 PRD domain and the FAD binding region of the eNOS reductase domains, respectively, and that dyn-2 PRD is sufficient to mediate dyn-2-dependent potentiation of eNOS activity, at least in part, by potentiating electron transfer.)	bind
18274	1	5934	7	NULL	NULL	NULL	NULL	dyn-2	GP		mediates			PRD		eNOS	GP	potentiation of;;activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_8_5894_s_13	12488320	(These data indicate that the binding domains of dyn-2 and eNOS reside within the dyn-2 PRD domain and the FAD binding region of the eNOS reductase domains, respectively, and that dyn-2 PRD is sufficient to mediate dyn-2-dependent potentiation of eNOS activity, at least in part, by potentiating electron transfer.)	bind
18275	2	5934	7	NULL	NULL	NULL	NULL	statement 1	Process		occur by					electron transfer	Process	potentiating			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_8_5894_s_13	12488320	(These data indicate that the binding domains of dyn-2 and eNOS reside within the dyn-2 PRD domain and the FAD binding region of the eNOS reductase domains, respectively, and that dyn-2 PRD is sufficient to mediate dyn-2-dependent potentiation of eNOS activity, at least in part, by potentiating electron transfer.)	bind
15415	1	5935	5	NULL	NULL	0	NULL	troponin	NULL	tropomyosin-truncated	bind	NULL				actin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_43_25455_s_126	7592713	(This calculation  uses the last data point of each curve in  Fig. 3 B.)  Removal of Ca   increased this ratio by a factor of  three in each case, suggesting a 3-fold effect of Ca   on tropomyosin-truncated troponin binding to actin.	bind
15416	2	5935	5	NULL	NULL	0	NULL	Ca	NULL		effect	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_43_25455_s_126	7592713	(This calculation  uses the last data point of each curve in  Fig. 3 B.)  Removal of Ca   increased this ratio by a factor of  three in each case, suggesting a 3-fold effect of Ca   on tropomyosin-truncated troponin binding to actin.	bind
18276	1	5935	7	NULL	NULL	NULL	NULL	troponin	GP	tropomyosin-truncated 	binds					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_43_25455_s_126	7592713	(This calculation  uses the last data point of each curve in  Fig. 3 B.)  Removal of Ca   increased this ratio by a factor of  three in each case, suggesting a 3-fold effect of Ca   on tropomyosin-truncated troponin binding to actin.	bind
44803	2	5935	7	NULL	NULL	NULL	NULL	Ca	Chemical		plays a role in					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_43_25455_s_126	7592713	(This calculation  uses the last data point of each curve in  Fig. 3 B.)  Removal of Ca   increased this ratio by a factor of  three in each case, suggesting a 3-fold effect of Ca   on tropomyosin-truncated troponin binding to actin.	bind
15419	1	5936	5	NULL	NULL	0	NULL	Int	NULL		bind	NULL	covalently			attP	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_5_11_1312_s_203	8574589	(This is in contrast to the situation with nicked suicide substrates, where unitary strand transfer is efficiently executed by displacement of an Int covalently bound to  attP by a hydroxyl from  attB  [11]  ; the difference between these situations is the subject of another study.)	bind
15420	2	5936	5	10	NULL	0	NULL	attB	NULL		bind	NULL		hydroxyl		attP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_5_11_1312_s_203	8574589	(This is in contrast to the situation with nicked suicide substrates, where unitary strand transfer is efficiently executed by displacement of an Int covalently bound to  attP by a hydroxyl from  attB  [11]  ; the difference between these situations is the subject of another study.)	bind
20343	3	5936	5	NULL	NULL	0	NULL	statement 2	NULL		displaces	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_5_11_1312_s_203	8574589	(This is in contrast to the situation with nicked suicide substrates, where unitary strand transfer is efficiently executed by displacement of an Int covalently bound to  attP by a hydroxyl from  attB  [11]  ; the difference between these situations is the subject of another study.)	bind
20344	4	5936	5	NULL	NULL	0	NULL	unitary strand transfer	NULL		executed by	NULL	efficiently			statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_5_11_1312_s_203	8574589	(This is in contrast to the situation with nicked suicide substrates, where unitary strand transfer is efficiently executed by displacement of an Int covalently bound to  attP by a hydroxyl from  attB  [11]  ; the difference between these situations is the subject of another study.)	bind
18277	1	5936	7	NULL	NULL	NULL	NULL	Int	GP		bind		covalently			attP	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_5_11_1312_s_203	8574589	(This is in contrast to the situation with nicked suicide substrates, where unitary strand transfer is efficiently executed by displacement of an Int covalently bound to  attP by a hydroxyl from  attB  [11]  ; the difference between these situations is the subject of another study.)	bind
18278	2	5936	7	NULL	NULL	NULL	NULL	attB	GP		binds			hydroxyl		attP	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_5_11_1312_s_203	8574589	(This is in contrast to the situation with nicked suicide substrates, where unitary strand transfer is efficiently executed by displacement of an Int covalently bound to  attP by a hydroxyl from  attB  [11]  ; the difference between these situations is the subject of another study.)	bind
18279	3	5936	7	NULL	NULL	NULL	NULL	statement 2	Process		displaces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_5_11_1312_s_203	8574589	(This is in contrast to the situation with nicked suicide substrates, where unitary strand transfer is efficiently executed by displacement of an Int covalently bound to  attP by a hydroxyl from  attB  [11]  ; the difference between these situations is the subject of another study.)	bind
18280	4	5936	7	NULL	NULL	NULL	NULL	unitary strand transfer	Process		is executed by		efficiently			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_5_11_1312_s_203	8574589	(This is in contrast to the situation with nicked suicide substrates, where unitary strand transfer is efficiently executed by displacement of an Int covalently bound to  attP by a hydroxyl from  attB  [11]  ; the difference between these situations is the subject of another study.)	bind
15421	1	5937	5	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				eIF2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_27_24697_s_181	11323413	(This material is free of eIF2, thus obviating the problem of GTP binding to any eIF2 present.)	bind
18281	1	5937	7	NULL	NULL	NULL	NULL	GTP	Chemical		binds					eIF2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_24697_s_181	11323413	(This material is free of eIF2, thus obviating the problem of GTP binding to any eIF2 present.)	bind
15422	1	5938	5	NULL	NULL	0	NULL	titin	NULL		bind	NULL		PEVK region		actin	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_99_8_795_s_42	17038648	(This region shares homology to the PEVK region of titin, which is known to bind to actin.	bind
18282	1	5938	7	NULL	NULL	NULL	NULL	titin	GP		binds to			PEVK region		actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_99_8_795_s_42	17038648	(This region shares homology to the PEVK region of titin, which is known to bind to actin.	bind
15423	1	5939	5	NULL	NULL	0	NULL	GroEL	NULL	single ring mutant	bind	NULL	rapidly			GroES 	NULL				NULL		0	NULL	NULL	NULL	gw60_structure_4_1_1_s_81	8805512	(This was shown by using a single ring mutant GroEL that rapidly binds but very slowly releases GroES in single turnover studies to trap released GroES; results revealed that a single turnover of ATPase was sufficient for productive release of OTC from  cis, but not  trans, complexes.)	bind
15424	2	5939	5	NULL	NULL	0	NULL	GroEL	NULL	single ring mutant	release	NULL	slowly			GroES	NULL				NULL		0	NULL	NULL	NULL	gw60_structure_4_1_1_s_81	8805512	(This was shown by using a single ring mutant GroEL that rapidly binds but very slowly releases GroES in single turnover studies to trap released GroES; results revealed that a single turnover of ATPase was sufficient for productive release of OTC from  cis, but not  trans, complexes.)	bind
15425	3	5939	5	NULL	NULL	0	NULL	ATPase	NULL	single turnover of	release	NULL	productively			OTC	NULL	from cis complex			NULL		NULL	NULL	NULL	NULL	gw60_structure_4_1_1_s_81	8805512	(This was shown by using a single ring mutant GroEL that rapidly binds but very slowly releases GroES in single turnover studies to trap released GroES; results revealed that a single turnover of ATPase was sufficient for productive release of OTC from  cis, but not  trans, complexes.)	bind
20345	4	5939	5	NULL	NULL	0	NULL	ATPase	NULL	single turnover of	does not release	NULL				OTC	NULL	from trans complex			NULL		NULL	NULL	NULL	NULL	gw60_structure_4_1_1_s_81	8805512	(This was shown by using a single ring mutant GroEL that rapidly binds but very slowly releases GroES in single turnover studies to trap released GroES; results revealed that a single turnover of ATPase was sufficient for productive release of OTC from  cis, but not  trans, complexes.)	bind
18283	1	5939	7	NULL	NULL	NULL	NULL	GroEL 	GP	single ring mutant	binds		rapidly			GroES	GP				NULL		NULL	NULL	NULL	NULL	gw60_structure_4_1_1_s_81	8805512	(This was shown by using a single ring mutant GroEL that rapidly binds but very slowly releases GroES in single turnover studies to trap released GroES; results revealed that a single turnover of ATPase was sufficient for productive release of OTC from  cis, but not  trans, complexes.)	bind
18284	2	5939	7	NULL	NULL	NULL	NULL	ATPase	GP	single turnover of 	release 		productively			OTC	GP	from cis complex			NULL		NULL	NULL	NULL	NULL	gw60_structure_4_1_1_s_81	8805512	(This was shown by using a single ring mutant GroEL that rapidly binds but very slowly releases GroES in single turnover studies to trap released GroES; results revealed that a single turnover of ATPase was sufficient for productive release of OTC from  cis, but not  trans, complexes.)	bind
18285	3	5939	7	NULL	NULL	NULL	NULL	ATPase	GP	single turnover of 	does not release		productively			OTC	GP	from trans complex			NULL		NULL	NULL	NULL	NULL	gw60_structure_4_1_1_s_81	8805512	(This was shown by using a single ring mutant GroEL that rapidly binds but very slowly releases GroES in single turnover studies to trap released GroES; results revealed that a single turnover of ATPase was sufficient for productive release of OTC from  cis, but not  trans, complexes.)	bind
20373	4	5939	7	NULL	NULL	NULL	NULL	GroEL	GP	single ring mutant	releases		slowly			GroES	GP				NULL		NULL	NULL	NULL	NULL	gw60_structure_4_1_1_s_81	8805512	(This was shown by using a single ring mutant GroEL that rapidly binds but very slowly releases GroES in single turnover studies to trap released GroES; results revealed that a single turnover of ATPase was sufficient for productive release of OTC from  cis, but not  trans, complexes.)	bind
15426	1	5941	5	NULL	NULL	0	NULL	Axin	NULL		bind	NULL				MEKK	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_269	12192039	(Top panel) In the absence of GSK-3beta, Axin binds MEKK, leading to activation of the JNK pathway.	bind
15427	2	5941	5	NULL	NULL	0	NULL	statement 1	NULL		in the absence of	NULL				GSK-3beta	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_269	12192039	(Top panel) In the absence of GSK-3beta, Axin binds MEKK, leading to activation of the JNK pathway.	bind
15428	3	5941	5	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				JNK pathway	NULL	activation of 			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_269	12192039	(Top panel) In the absence of GSK-3beta, Axin binds MEKK, leading to activation of the JNK pathway.	bind
18288	1	5941	7	NULL	NULL	NULL	NULL	Axin	GP		binds					MEKK	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_269	12192039	(Top panel) In the absence of GSK-3beta, Axin binds MEKK, leading to activation of the JNK pathway.	bind
18289	2	5941	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs in the absence of					GSK-3beta	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_269	12192039	(Top panel) In the absence of GSK-3beta, Axin binds MEKK, leading to activation of the JNK pathway.	bind
18290	3	5941	7	NULL	NULL	NULL	NULL	statement 1	Process		leads to					JNK pathway	Process	activation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_269	12192039	(Top panel) In the absence of GSK-3beta, Axin binds MEKK, leading to activation of the JNK pathway.	bind
15429	1	5942	5	NULL	NULL	0	NULL	Axin	NULL		bind	NULL				beta-catenin	NULL	free			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_263	12192039	(Top panel) In the absence of HIC or I-mfa, Axin binds free beta-catenin or beta-catenin that is released from E-cadherin and promotes phosphorylation of beta-catenin by GSK-3beta and beta-catenin degradation.	bind
15430	2	5942	5	NULL	NULL	0	NULL	statement 1	NULL		in the absence of	NULL				HIC	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_263	12192039	(Top panel) In the absence of HIC or I-mfa, Axin binds free beta-catenin or beta-catenin that is released from E-cadherin and promotes phosphorylation of beta-catenin by GSK-3beta and beta-catenin degradation.	bind
15431	3	5942	5	NULL	NULL	0	NULL	statement 1	NULL		in the absence of	NULL				I-mfa	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_263	12192039	(Top panel) In the absence of HIC or I-mfa, Axin binds free beta-catenin or beta-catenin that is released from E-cadherin and promotes phosphorylation of beta-catenin by GSK-3beta and beta-catenin degradation.	bind
15432	4	5942	5	NULL	NULL	0	NULL	statement 2	NULL		is an alternative to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_263	12192039	(Top panel) In the absence of HIC or I-mfa, Axin binds free beta-catenin or beta-catenin that is released from E-cadherin and promotes phosphorylation of beta-catenin by GSK-3beta and beta-catenin degradation.	bind
15433	5	5942	5	NULL	NULL	0	NULL	beta-catenin	NULL		is released from	NULL				E-cadherin	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_263	12192039	(Top panel) In the absence of HIC or I-mfa, Axin binds free beta-catenin or beta-catenin that is released from E-cadherin and promotes phosphorylation of beta-catenin by GSK-3beta and beta-catenin degradation.	bind
15434	6	5942	5	NULL	NULL	0	NULL	Axin	NULL		bind	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_263	12192039	(Top panel) In the absence of HIC or I-mfa, Axin binds free beta-catenin or beta-catenin that is released from E-cadherin and promotes phosphorylation of beta-catenin by GSK-3beta and beta-catenin degradation.	bind
15435	7	5942	5	NULL	NULL	0	NULL	statement 6	NULL		in the absence of	NULL				HIC	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_263	12192039	(Top panel) In the absence of HIC or I-mfa, Axin binds free beta-catenin or beta-catenin that is released from E-cadherin and promotes phosphorylation of beta-catenin by GSK-3beta and beta-catenin degradation.	bind
15436	8	5942	5	NULL	NULL	0	NULL	statement 6	NULL		in the absence of	NULL				I-mfa	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_263	12192039	(Top panel) In the absence of HIC or I-mfa, Axin binds free beta-catenin or beta-catenin that is released from E-cadherin and promotes phosphorylation of beta-catenin by GSK-3beta and beta-catenin degradation.	bind
15437	9	5942	5	NULL	NULL	0	NULL	statement 7	NULL		is an alternative to	NULL				statement 8	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_263	12192039	(Top panel) In the absence of HIC or I-mfa, Axin binds free beta-catenin or beta-catenin that is released from E-cadherin and promotes phosphorylation of beta-catenin by GSK-3beta and beta-catenin degradation.	bind
15438	10	5942	5	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_263	12192039	(Top panel) In the absence of HIC or I-mfa, Axin binds free beta-catenin or beta-catenin that is released from E-cadherin and promotes phosphorylation of beta-catenin by GSK-3beta and beta-catenin degradation.	bind
15439	11	5942	5	NULL	NULL	0	NULL	Axin	NULL		promote	NULL				beta-catenin	NULL	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_263	12192039	(Top panel) In the absence of HIC or I-mfa, Axin binds free beta-catenin or beta-catenin that is released from E-cadherin and promotes phosphorylation of beta-catenin by GSK-3beta and beta-catenin degradation.	bind
15440	12	5942	5	NULL	NULL	0	NULL	GSK-3beta	NULL		undergoes	NULL				degradation	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_263	12192039	(Top panel) In the absence of HIC or I-mfa, Axin binds free beta-catenin or beta-catenin that is released from E-cadherin and promotes phosphorylation of beta-catenin by GSK-3beta and beta-catenin degradation.	bind
15441	13	5942	5	NULL	NULL	0	NULL	beta-catenin	NULL		undergoes	NULL				degradation	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_263	12192039	(Top panel) In the absence of HIC or I-mfa, Axin binds free beta-catenin or beta-catenin that is released from E-cadherin and promotes phosphorylation of beta-catenin by GSK-3beta and beta-catenin degradation.	bind
15442	14	5942	5	NULL	NULL	0	NULL	statement 12	NULL		leads to	NULL				statement 11	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_263	12192039	(Top panel) In the absence of HIC or I-mfa, Axin binds free beta-catenin or beta-catenin that is released from E-cadherin and promotes phosphorylation of beta-catenin by GSK-3beta and beta-catenin degradation.	bind
15443	15	5942	5	NULL	NULL	0	NULL	statement 13	NULL		leads to	NULL				statement 11	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_263	12192039	(Top panel) In the absence of HIC or I-mfa, Axin binds free beta-catenin or beta-catenin that is released from E-cadherin and promotes phosphorylation of beta-catenin by GSK-3beta and beta-catenin degradation.	bind
18291	1	5942	7	NULL	NULL	NULL	NULL	Axin	GP		binds					beta-catenin	GP	free			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_263	12192039	(Top panel) In the absence of HIC or I-mfa, Axin binds free beta-catenin or beta-catenin that is released from E-cadherin and promotes phosphorylation of beta-catenin by GSK-3beta and beta-catenin degradation.	bind
18292	2	5942	7	NULL	NULL	NULL	NULL	E-cadherin	GP		release					beta-catenin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_263	12192039	(Top panel) In the absence of HIC or I-mfa, Axin binds free beta-catenin or beta-catenin that is released from E-cadherin and promotes phosphorylation of beta-catenin by GSK-3beta and beta-catenin degradation.	bind
18293	3	5942	7	NULL	NULL	NULL	NULL	Axin	GP		binds					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_263	12192039	(Top panel) In the absence of HIC or I-mfa, Axin binds free beta-catenin or beta-catenin that is released from E-cadherin and promotes phosphorylation of beta-catenin by GSK-3beta and beta-catenin degradation.	bind
18294	4	5942	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs in the absence of					HIC	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_263	12192039	(Top panel) In the absence of HIC or I-mfa, Axin binds free beta-catenin or beta-catenin that is released from E-cadherin and promotes phosphorylation of beta-catenin by GSK-3beta and beta-catenin degradation.	bind
18295	5	5942	7	NULL	NULL	NULL	NULL	statement 3	Process		occurs in the absence of					HIC	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_263	12192039	(Top panel) In the absence of HIC or I-mfa, Axin binds free beta-catenin or beta-catenin that is released from E-cadherin and promotes phosphorylation of beta-catenin by GSK-3beta and beta-catenin degradation.	bind
18296	6	5942	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs in the absence of					I-mfa	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_263	12192039	(Top panel) In the absence of HIC or I-mfa, Axin binds free beta-catenin or beta-catenin that is released from E-cadherin and promotes phosphorylation of beta-catenin by GSK-3beta and beta-catenin degradation.	bind
18297	7	5942	7	NULL	NULL	NULL	NULL	statement 3	Process		occurs in the absence of					I-mfa	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_263	12192039	(Top panel) In the absence of HIC or I-mfa, Axin binds free beta-catenin or beta-catenin that is released from E-cadherin and promotes phosphorylation of beta-catenin by GSK-3beta and beta-catenin degradation.	bind
18298	8	5942	7	NULL	NULL	NULL	NULL	GSK-3beta 	GP		phosphorylates					beta-catenin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_263	12192039	(Top panel) In the absence of HIC or I-mfa, Axin binds free beta-catenin or beta-catenin that is released from E-cadherin and promotes phosphorylation of beta-catenin by GSK-3beta and beta-catenin degradation.	bind
18299	9	5942	7	NULL	NULL	NULL	NULL	statement 1	Process		promotes					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_263	12192039	(Top panel) In the absence of HIC or I-mfa, Axin binds free beta-catenin or beta-catenin that is released from E-cadherin and promotes phosphorylation of beta-catenin by GSK-3beta and beta-catenin degradation.	bind
18300	10	5942	7	NULL	NULL	NULL	NULL	statement 3	Process		promotes					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_263	12192039	(Top panel) In the absence of HIC or I-mfa, Axin binds free beta-catenin or beta-catenin that is released from E-cadherin and promotes phosphorylation of beta-catenin by GSK-3beta and beta-catenin degradation.	bind
18301	11	5942	7	NULL	NULL	NULL	NULL	statement 1	Process		promotes					beta-catenin	Process	degradation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_263	12192039	(Top panel) In the absence of HIC or I-mfa, Axin binds free beta-catenin or beta-catenin that is released from E-cadherin and promotes phosphorylation of beta-catenin by GSK-3beta and beta-catenin degradation.	bind
18302	12	5942	7	NULL	NULL	NULL	NULL	statement 3	Process		promotes					beta-catenin	GP	degradation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6393_s_263	12192039	(Top panel) In the absence of HIC or I-mfa, Axin binds free beta-catenin or beta-catenin that is released from E-cadherin and promotes phosphorylation of beta-catenin by GSK-3beta and beta-catenin degradation.	bind
15444	1	5944	5	NULL	NULL	0	NULL	Ets-1	NULL		bind	NULL				EBS probe	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_20_4154_s_168	11600704	(Top) EMSA of Ets-1 binding to the EBS probe.	bind
18304	1	5944	7	NULL	NULL	NULL	NULL	Ets-1	GP		binds to					EBS probe	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_20_4154_s_168	11600704	(Top) EMSA of Ets-1 binding to the EBS probe.	bind
15445	1	5945	5	NULL	NULL	0	NULL	SAP1a	NULL		bind	NULL				EBS probe	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_20_4154_s_130	11600704	(Top) EMSA of SAP1a binding to the EBS probe.	bind
18305	1	5945	7	NULL	NULL	NULL	NULL	SAP1a	GP		bind					EBS probe	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_20_4154_s_130	11600704	(Top) EMSA of SAP1a binding to the EBS probe.	bind
15446	1	5946	5	NULL	NULL	0	NULL	LR1	NULL		bind	NULL				pBEND2(Sgamma1)	NULL			164 bp fragments	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_14_2651_s_89	10908319	(Top) Gel mobility shift assay of LR1 binding to 164 bp fragments of pBEND2(Sgamma1) with the LR1 site at permuted positions, as indicated above; this corresponds to digestion with:	bind
46296	2	5946	5	NULL	NULL	0	NULL		NULL		resides within	NULL			LR1 site		NULL			164 bp fragments	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_14_2651_s_89	10908319	(Top) Gel mobility shift assay of LR1 binding to 164 bp fragments of pBEND2(Sgamma1) with the LR1 site at permuted positions, as indicated above; this corresponds to digestion with:	bind
18306	1	5946	7	NULL	NULL	NULL	NULL	LR1	GP		bind					pBEND2(Sgamma1)	GP			164 bp fragments 	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_14_2651_s_89	10908319	(Top) Gel mobility shift assay of LR1 binding to 164 bp fragments of pBEND2(Sgamma1) with the LR1 site at permuted positions, as indicated above; this corresponds to digestion with:	bind
18330	2	5946	7	NULL	NULL	0	NULL		NULL		resides within	NULL			LR1 site		NULL			164 bp fragments	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_14_2651_s_89	10908319	(Top) Gel mobility shift assay of LR1 binding to 164 bp fragments of pBEND2(Sgamma1) with the LR1 site at permuted positions, as indicated above; this corresponds to digestion with:	bind
15447	1	5950	5	NULL	NULL	0	NULL	NuMA	NULL		associate with	NULL				dynein	NULL	cytoplasmic			NULL		0	NULL	NULL	NULL	gw60_cell_87_3_447_s_188	8898198	(Top) NuMA associates with cytoplasmic dynein; its binding to stationary microtubules enables the  complex to translocate free microtubules towards the chromatin or, by binding to free  microtubules, to move them polewards.	bind
15448	2	5950	5	NULL	NULL	0	NULL	NuMA	NULL		bind	NULL				microtubules	NULL	stationary			NULL		0	NULL	NULL	NULL	gw60_cell_87_3_447_s_188	8898198	(Top) NuMA associates with cytoplasmic dynein; its binding to stationary microtubules enables the  complex to translocate free microtubules towards the chromatin or, by binding to free  microtubules, to move them polewards.	bind
15449	3	5950	5	NULL	NULL	0	NULL	statement 1	NULL		translocates	NULL				free microtubules	NULL	towards chromatin			NULL		NULL	NULL	NULL	NULL	gw60_cell_87_3_447_s_188	8898198	(Top) NuMA associates with cytoplasmic dynein; its binding to stationary microtubules enables the  complex to translocate free microtubules towards the chromatin or, by binding to free  microtubules, to move them polewards.	bind
15450	4	5950	5	NULL	NULL	0	NULL	statement 2	NULL		enables	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_87_3_447_s_188	8898198	(Top) NuMA associates with cytoplasmic dynein; its binding to stationary microtubules enables the  complex to translocate free microtubules towards the chromatin or, by binding to free  microtubules, to move them polewards.	bind
15451	5	5950	5	NULL	NULL	0	NULL	NuMA	NULL		bind	NULL				microtubules	NULL	free			NULL		0	NULL	NULL	NULL	gw60_cell_87_3_447_s_188	8898198	(Top) NuMA associates with cytoplasmic dynein; its binding to stationary microtubules enables the  complex to translocate free microtubules towards the chromatin or, by binding to free  microtubules, to move them polewards.	bind
15452	6	5950	5	NULL	NULL	0	NULL	statement 5	NULL		moves	NULL				free microtubules	NULL	polewards			NULL		0	NULL	NULL	NULL	gw60_cell_87_3_447_s_188	8898198	(Top) NuMA associates with cytoplasmic dynein; its binding to stationary microtubules enables the  complex to translocate free microtubules towards the chromatin or, by binding to free  microtubules, to move them polewards.	bind
18331	1	5950	7	NULL	NULL	NULL	NULL	NuMA	GP		binds					dynein	GP	cytoplasmic			NULL		NULL	NULL	NULL	NULL	gw60_cell_87_3_447_s_188	8898198	(Top) NuMA associates with cytoplasmic dynein; its binding to stationary microtubules enables the  complex to translocate free microtubules towards the chromatin or, by binding to free  microtubules, to move them polewards.	bind
18332	2	5950	7	NULL	NULL	NULL	NULL	statement 1	Process		binds					 microtubules	CellComponent	stationary			NULL		NULL	NULL	NULL	NULL	gw60_cell_87_3_447_s_188	8898198	(Top) NuMA associates with cytoplasmic dynein; its binding to stationary microtubules enables the  complex to translocate free microtubules towards the chromatin or, by binding to free  microtubules, to move them polewards.	bind
18333	3	5950	7	NULL	NULL	NULL	NULL	statement 1	Process		translocate					free microtubules	CellComponent	 towards chromatin			NULL		NULL	NULL	NULL	NULL	gw60_cell_87_3_447_s_188	8898198	(Top) NuMA associates with cytoplasmic dynein; its binding to stationary microtubules enables the  complex to translocate free microtubules towards the chromatin or, by binding to free  microtubules, to move them polewards.	bind
18334	4	5950	7	NULL	NULL	NULL	NULL	statement 2	Process		enables					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_87_3_447_s_188	8898198	(Top) NuMA associates with cytoplasmic dynein; its binding to stationary microtubules enables the  complex to translocate free microtubules towards the chromatin or, by binding to free  microtubules, to move them polewards.	bind
18335	5	5950	7	NULL	NULL	NULL	NULL	statement 1	Process		binds					free microtubules	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cell_87_3_447_s_188	8898198	(Top) NuMA associates with cytoplasmic dynein; its binding to stationary microtubules enables the  complex to translocate free microtubules towards the chromatin or, by binding to free  microtubules, to move them polewards.	bind
18336	6	5950	7	NULL	NULL	NULL	NULL	statement 5	Process		move 					free microtubles	CellComponent	poleward			NULL		NULL	NULL	NULL	NULL	gw60_cell_87_3_447_s_188	8898198	(Top) NuMA associates with cytoplasmic dynein; its binding to stationary microtubules enables the  complex to translocate free microtubules towards the chromatin or, by binding to free  microtubules, to move them polewards.	bind
15453	1	5951	5	NULL	NULL	0	NULL	Rho	NULL		bind	NULL					NULL		RBD		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_158_1_153_s_87	12105187	(Top) Rho bound to RBD.	bind
18337	1	5951	7	NULL	NULL	NULL	NULL	Rho	GP		bind								RBD		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_158_1_153_s_87	12105187	(Top) Rho bound to RBD.	bind
15454	1	5953	5	NULL	NULL	0	NULL	S3P	NULL		bind	NULL				EPSP synthase	NULL				NULL		0	NULL	NULL	NULL	gw70_febslett_579_25_5773_s_105	16225867	(Top): S3P and glyphosate bound to EPSP synthase  (PDB 1G6S).	bind
20346	2	5953	5	NULL	NULL	0	NULL	glyphosate	NULL		bind	NULL				EPSP synthase	NULL				NULL		0	NULL	NULL	NULL	gw70_febslett_579_25_5773_s_105	16225867	(Top): S3P and glyphosate bound to EPSP synthase  (PDB 1G6S).	bind
18338	1	5953	7	NULL	NULL	NULL	NULL	S3P	GP		bind					EPSP synthase	GP				NULL		NULL	NULL	NULL	NULL	gw70_febslett_579_25_5773_s_105	16225867	(Top): S3P and glyphosate bound to EPSP synthase  (PDB 1G6S).	bind
18339	2	5953	7	NULL	NULL	NULL	NULL	glyphosate	Chemical		bind					EPSP synthase 	GP				NULL		NULL	NULL	NULL	NULL	gw70_febslett_579_25_5773_s_105	16225867	(Top): S3P and glyphosate bound to EPSP synthase  (PDB 1G6S).	bind
15455	1	5954	5	NULL	NULL	0	NULL	S3P	NULL		bind	NULL				EPSP synthase	NULL				NULL		0	NULL	NULL	NULL	gw70_febslett_579_25_5773_s_81	16225867	(Top): S3P bound to EPSP synthase (PDB 1G6T).	bind
18340	1	5954	7	NULL	NULL	NULL	NULL	S3P	GP		bind					EPSP synthase	GP				NULL		NULL	NULL	NULL	NULL	gw70_febslett_579_25_5773_s_81	16225867	(Top): S3P bound to EPSP synthase (PDB 1G6T).	bind
16380	1	5955	5	NULL	NULL	0	NULL	RNA polymerase II	NULL		bind	NULL	relatively poorly			GST-Myc	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_22_20405_s_86	12660246	(TRAPs 240, 230, and 170), RNA  polymerase II, and the general transcription factor TFIIB bound relatively  poorly to GST-Myc and GST-MycN263 ( i.e. binding was either  undetectable or well below 5% of the input in corresponding panels in   lanes 3 and  6).	bind
16381	2	5955	5	NULL	NULL	0	NULL	RNA polymerase II	NULL		bind	NULL	relatively poorly			GST-Myc	NULL		N263		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_22_20405_s_86	12660246	(TRAPs 240, 230, and 170), RNA  polymerase II, and the general transcription factor TFIIB bound relatively  poorly to GST-Myc and GST-MycN263 ( i.e. binding was either  undetectable or well below 5% of the input in corresponding panels in   lanes 3 and  6).	bind
16382	3	5955	5	10	NULL	0	NULL	TFIIB	NULL		bind	NULL	relatively poorly			GST-Myc	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_20405_s_86	12660246	(TRAPs 240, 230, and 170), RNA  polymerase II, and the general transcription factor TFIIB bound relatively  poorly to GST-Myc and GST-MycN263 ( i.e. binding was either  undetectable or well below 5% of the input in corresponding panels in   lanes 3 and  6).	bind
16383	4	5955	5	10	NULL	0	NULL	TFIIB	NULL		bind	NULL	relatively poorly			GST-Myc	NULL		N263		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_20405_s_86	12660246	(TRAPs 240, 230, and 170), RNA  polymerase II, and the general transcription factor TFIIB bound relatively  poorly to GST-Myc and GST-MycN263 ( i.e. binding was either  undetectable or well below 5% of the input in corresponding panels in   lanes 3 and  6).	bind
20347	5	5955	5	NULL	NULL	0	NULL	TRAP 240	NULL		bind	NULL	relatively poorly			GST-Myc	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_22_20405_s_86	12660246	(TRAPs 240, 230, and 170), RNA  polymerase II, and the general transcription factor TFIIB bound relatively  poorly to GST-Myc and GST-MycN263 ( i.e. binding was either  undetectable or well below 5% of the input in corresponding panels in   lanes 3 and  6).	bind
20348	6	5955	5	NULL	NULL	0	NULL	TRAP 240	NULL		bind	NULL	relatively poorly			GST-Myc	NULL		N263		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_22_20405_s_86	12660246	(TRAPs 240, 230, and 170), RNA  polymerase II, and the general transcription factor TFIIB bound relatively  poorly to GST-Myc and GST-MycN263 ( i.e. binding was either  undetectable or well below 5% of the input in corresponding panels in   lanes 3 and  6).	bind
20349	7	5955	5	NULL	NULL	0	NULL	TRAP 230	NULL		bind	NULL	relatively poorly			GST-Myc	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_22_20405_s_86	12660246	(TRAPs 240, 230, and 170), RNA  polymerase II, and the general transcription factor TFIIB bound relatively  poorly to GST-Myc and GST-MycN263 ( i.e. binding was either  undetectable or well below 5% of the input in corresponding panels in   lanes 3 and  6).	bind
20350	8	5955	5	NULL	NULL	0	NULL	TRAP 230	NULL		bind	NULL	relatively poorly			GST-Myc	NULL		N263		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_22_20405_s_86	12660246	(TRAPs 240, 230, and 170), RNA  polymerase II, and the general transcription factor TFIIB bound relatively  poorly to GST-Myc and GST-MycN263 ( i.e. binding was either  undetectable or well below 5% of the input in corresponding panels in   lanes 3 and  6).	bind
20351	9	5955	5	NULL	NULL	0	NULL	TRAP 170	NULL		bind	NULL	relatively poorly			GST-Myc	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_22_20405_s_86	12660246	(TRAPs 240, 230, and 170), RNA  polymerase II, and the general transcription factor TFIIB bound relatively  poorly to GST-Myc and GST-MycN263 ( i.e. binding was either  undetectable or well below 5% of the input in corresponding panels in   lanes 3 and  6).	bind
20352	10	5955	5	NULL	NULL	0	NULL	TRAP 170	NULL		bind	NULL	relatively poorly			GST-Myc	NULL		N263		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_22_20405_s_86	12660246	(TRAPs 240, 230, and 170), RNA  polymerase II, and the general transcription factor TFIIB bound relatively  poorly to GST-Myc and GST-MycN263 ( i.e. binding was either  undetectable or well below 5% of the input in corresponding panels in   lanes 3 and  6).	bind
44804	11	5955	5	10	NULL	0	NULL	TFIIB	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_22_20405_s_86	12660246	(TRAPs 240, 230, and 170), RNA  polymerase II, and the general transcription factor TFIIB bound relatively  poorly to GST-Myc and GST-MycN263 ( i.e. binding was either  undetectable or well below 5% of the input in corresponding panels in   lanes 3 and  6).	bind
18341	1	5955	7	NULL	NULL	NULL	NULL	TRAP 240	GP		bind		poorly			GST-Myc	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_20405_s_86	12660246	(TRAPs 240, 230, and 170), RNA  polymerase II, and the general transcription factor TFIIB bound relatively  poorly to GST-Myc and GST-MycN263 ( i.e. binding was either  undetectable or well below 5% of the input in corresponding panels in   lanes 3 and  6).	bind
18342	2	5955	7	NULL	NULL	NULL	NULL	TRAP 240	GP		bind		poorly			GST-Myc	GP		N263		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_20405_s_86	12660246	(TRAPs 240, 230, and 170), RNA  polymerase II, and the general transcription factor TFIIB bound relatively  poorly to GST-Myc and GST-MycN263 ( i.e. binding was either  undetectable or well below 5% of the input in corresponding panels in   lanes 3 and  6).	bind
18343	3	5955	7	NULL	NULL	NULL	NULL	TRAP 230	GP		bind		poorly			GST-Myc	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_20405_s_86	12660246	(TRAPs 240, 230, and 170), RNA  polymerase II, and the general transcription factor TFIIB bound relatively  poorly to GST-Myc and GST-MycN263 ( i.e. binding was either  undetectable or well below 5% of the input in corresponding panels in   lanes 3 and  6).	bind
18344	4	5955	7	NULL	NULL	NULL	NULL	TRAP 230	GP		bind		poorly			GST-Myc	GP		N263		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_20405_s_86	12660246	(TRAPs 240, 230, and 170), RNA  polymerase II, and the general transcription factor TFIIB bound relatively  poorly to GST-Myc and GST-MycN263 ( i.e. binding was either  undetectable or well below 5% of the input in corresponding panels in   lanes 3 and  6).	bind
18345	5	5955	7	NULL	NULL	NULL	NULL	TRAP 170	GP		bind		poorly			GST-Myc	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_20405_s_86	12660246	(TRAPs 240, 230, and 170), RNA  polymerase II, and the general transcription factor TFIIB bound relatively  poorly to GST-Myc and GST-MycN263 ( i.e. binding was either  undetectable or well below 5% of the input in corresponding panels in   lanes 3 and  6).	bind
18346	6	5955	7	NULL	NULL	NULL	NULL	TRAP 170	GP		bind		poorly			GST-Myc	GP		N263		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_20405_s_86	12660246	(TRAPs 240, 230, and 170), RNA  polymerase II, and the general transcription factor TFIIB bound relatively  poorly to GST-Myc and GST-MycN263 ( i.e. binding was either  undetectable or well below 5% of the input in corresponding panels in   lanes 3 and  6).	bind
18347	7	5955	7	NULL	NULL	NULL	NULL	RNA polymerase II	GP		bind		poorly			GST-Myc	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_20405_s_86	12660246	(TRAPs 240, 230, and 170), RNA  polymerase II, and the general transcription factor TFIIB bound relatively  poorly to GST-Myc and GST-MycN263 ( i.e. binding was either  undetectable or well below 5% of the input in corresponding panels in   lanes 3 and  6).	bind
18348	8	5955	7	NULL	NULL	NULL	NULL	RNA polymerase II	GP		bind		poorly			GST-Myc	GP		N263		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_20405_s_86	12660246	(TRAPs 240, 230, and 170), RNA  polymerase II, and the general transcription factor TFIIB bound relatively  poorly to GST-Myc and GST-MycN263 ( i.e. binding was either  undetectable or well below 5% of the input in corresponding panels in   lanes 3 and  6).	bind
18349	9	5955	7	NULL	NULL	NULL	NULL	TFIIB	GP		bind		poorly			GST-Myc	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_20405_s_86	12660246	(TRAPs 240, 230, and 170), RNA  polymerase II, and the general transcription factor TFIIB bound relatively  poorly to GST-Myc and GST-MycN263 ( i.e. binding was either  undetectable or well below 5% of the input in corresponding panels in   lanes 3 and  6).	bind
18350	10	5955	7	NULL	NULL	NULL	NULL	TFIIB	GP		bind		poorly			GST-Myc	GP		N263		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_20405_s_86	12660246	(TRAPs 240, 230, and 170), RNA  polymerase II, and the general transcription factor TFIIB bound relatively  poorly to GST-Myc and GST-MycN263 ( i.e. binding was either  undetectable or well below 5% of the input in corresponding panels in   lanes 3 and  6).	bind
44805	11	5955	7	NULL	NULL	NULL	NULL	TFIIB	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_20405_s_86	12660246	(TRAPs 240, 230, and 170), RNA  polymerase II, and the general transcription factor TFIIB bound relatively  poorly to GST-Myc and GST-MycN263 ( i.e. binding was either  undetectable or well below 5% of the input in corresponding panels in   lanes 3 and  6).	bind
15456	1	5956	5	NULL	NULL	0	NULL	seven-transmembrane domain superfamily receptor	NULL		bind	NULL				RANTES	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_13_7551_s_27	8631787	(Type A and Type  B( 17,  18) ) and a single receptor that binds both  RANTES and MIP-1alpha  ( 19,  20) have been cloned and  shown to be members of the seven-transmembrane domain superfamily of  receptors.	bind
15457	2	5956	5	NULL	NULL	0	NULL	seven-transmembrane domain superfamily receptor	NULL		bind	NULL				MIP-1alpha	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_13_7551_s_27	8631787	(Type A and Type  B( 17,  18) ) and a single receptor that binds both  RANTES and MIP-1alpha  ( 19,  20) have been cloned and  shown to be members of the seven-transmembrane domain superfamily of  receptors.	bind
18351	1	5956	7	NULL	NULL	NULL	NULL	seven-transmembrane domain superfamily receptor	GP		bind					RANTES	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_13_7551_s_27	8631787	(Type A and Type  B( 17,  18) ) and a single receptor that binds both  RANTES and MIP-1alpha  ( 19,  20) have been cloned and  shown to be members of the seven-transmembrane domain superfamily of  receptors.	bind
18352	2	5956	7	NULL	NULL	NULL	NULL	seven-transmembrane domain superfamily receptor	GP		bind					MIP-1alpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_13_7551_s_27	8631787	(Type A and Type  B( 17,  18) ) and a single receptor that binds both  RANTES and MIP-1alpha  ( 19,  20) have been cloned and  shown to be members of the seven-transmembrane domain superfamily of  receptors.	bind
18353	1	5957	7	NULL	NULL	NULL	NULL	 		conservative mutations	abolish			Glu327Gln 		Tl+ ion	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1505_1_57_s_104	11248189	(Upper left) High affinity 204Tl+ in wild type (WT) ( ) with maximum capacity 1.9 plus-or-minus 0.3 Tl+ ions per ouabain binding site and  K1/2=7.3 plus-or-minus 3.3  M. Tl+ ion binding is abolished after conservative mutations Glu327Gln ( ) or Glu327Asp ( ).	bind
18354	2	5957	7	NULL	NULL	NULL	NULL			conservative mutations	abolish			Glu327Asp		Tl+ ion	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1505_1_57_s_104	11248189	(Upper left) High affinity 204Tl+ in wild type (WT) ( ) with maximum capacity 1.9 plus-or-minus 0.3 Tl+ ions per ouabain binding site and  K1/2=7.3 plus-or-minus 3.3  M. Tl+ ion binding is abolished after conservative mutations Glu327Gln ( ) or Glu327Asp ( ).	bind
15458	1	5958	5	NULL	NULL	0	NULL	SKAP55	NULL		bind	NULL				FYB	NULL		SH3 domain		NULL	in vivo	NULL	NULL	NULL	NULL	gw60_embo_19_12_2889_s_110	10856234	(Upper panel) Mutation of tyrosine residues Y294F/Y297F attenuates  in vivo SKAP55 binding to the FYB SH3 domain.	bind
15459	2	5958	5	NULL	NULL	0	NULL		NULL	mutant	attenuate	NULL		Y294F/Y297F		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_19_12_2889_s_110	10856234	(Upper panel) Mutation of tyrosine residues Y294F/Y297F attenuates  in vivo SKAP55 binding to the FYB SH3 domain.	bind
18355	1	5958	7	NULL	NULL	NULL	NULL	SKAP55	GP		bind					FYB	GP		SH3 domain		NULL	in vivo	NULL	NULL	NULL	NULL	gw60_embo_19_12_2889_s_110	10856234	(Upper panel) Mutation of tyrosine residues Y294F/Y297F attenuates  in vivo SKAP55 binding to the FYB SH3 domain.	bind
18356	2	5958	7	NULL	NULL	NULL	NULL	tyrosine residues	AminoAcid	mutation of 	attenuate			Y294F/Y297F		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_12_2889_s_110	10856234	(Upper panel) Mutation of tyrosine residues Y294F/Y297F attenuates  in vivo SKAP55 binding to the FYB SH3 domain.	bind
15460	1	5959	5	NULL	NULL	0	NULL	PABP	NULL		bind	NULL				Cp transcript	NULL	endogenous			NULL	in U937 cells	0	NULL	NULL	NULL	gw60_molcellbiol_21_19_6440_s_264	11533233	(Upper panel) The binding of PABP to endogenous Cp transcript in U937 cells was determined.	bind
18358	1	5959	7	NULL	NULL	NULL	NULL	PABP	GP		bind					Cp transcript 	GP	endogenous			NULL	U937 cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_19_6440_s_264	11533233	(Upper panel) The binding of PABP to endogenous Cp transcript in U937 cells was determined.	bind
15461	1	5961	5	10	NULL	0	NULL	gD		soluble;; recombinant	bind								C-C'-C"` beta-strands		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_30_27006_s_49	12011057	(v) A soluble recombinant form of gD that binds to the C-C'-C"` beta-strands interfered with the binding of nectin3 and nectin4 to nectin1.	bind
15462	2	5961	5	NULL	NULL	0	NULL	nectin3	NULL		bind	NULL				nectin1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_30_27006_s_49	12011057	(v) A soluble recombinant form of gD that binds to the C-C'-C"` beta-strands interfered with the binding of nectin3 and nectin4 to nectin1.	bind
15463	3	5961	5	NULL	NULL	0	NULL	nectin4	NULL		bind	NULL				nectin1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_30_27006_s_49	12011057	(v) A soluble recombinant form of gD that binds to the C-C'-C"` beta-strands interfered with the binding of nectin3 and nectin4 to nectin1.	bind
15464	4	5961	5	NULL	NULL	0	NULL	statement 1	NULL		interfere with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_30_27006_s_49	12011057	(v) A soluble recombinant form of gD that binds to the C-C'-C"` beta-strands interfered with the binding of nectin3 and nectin4 to nectin1.	bind
15465	5	5961	5	NULL	NULL	0	NULL	statement 1	NULL		interfere with	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_30_27006_s_49	12011057	(v) A soluble recombinant form of gD that binds to the C-C'-C"` beta-strands interfered with the binding of nectin3 and nectin4 to nectin1.	bind
18359	1	5961	7	NULL	NULL	NULL	NULL	gD	GP	soluble;; recombinant	binds to								C-C'-C"` beta-strands		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_30_27006_s_49	12011057	(v) A soluble recombinant form of gD that binds to the C-C'-C"` beta-strands interfered with the binding of nectin3 and nectin4 to nectin1.	bind
18360	2	5961	7	NULL	NULL	NULL	NULL	nectin3	GP		bind					nectin1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_30_27006_s_49	12011057	(v) A soluble recombinant form of gD that binds to the C-C'-C"` beta-strands interfered with the binding of nectin3 and nectin4 to nectin1.	bind
18361	3	5961	7	NULL	NULL	NULL	NULL	nectin4	GP		bind					nectin1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_30_27006_s_49	12011057	(v) A soluble recombinant form of gD that binds to the C-C'-C"` beta-strands interfered with the binding of nectin3 and nectin4 to nectin1.	bind
18362	4	5961	7	NULL	NULL	NULL	NULL	statement 1	Process		interferes with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_30_27006_s_49	12011057	(v) A soluble recombinant form of gD that binds to the C-C'-C"` beta-strands interfered with the binding of nectin3 and nectin4 to nectin1.	bind
18363	5	5961	7	NULL	NULL	NULL	NULL	statement 1	Process		interferes with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_30_27006_s_49	12011057	(v) A soluble recombinant form of gD that binds to the C-C'-C"` beta-strands interfered with the binding of nectin3 and nectin4 to nectin1.	bind
15466	1	5962	5	NULL	NULL	0	NULL	KaiA	NULL		bind	NULL	exclusively			CII half 	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_25_9_2017_s_268	16628225	(v) EM and mutational data are consistent with KaiA binding exclusively to the  CII half (this work).	bind
18364	1	5962	7	NULL	NULL	NULL	NULL	KaiA	GP		bind		exclusively			CII half	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_9_2017_s_268	16628225	(v) EM and mutational data are consistent with KaiA binding exclusively to the  CII half (this work).	bind
20353	1	5963	5	NULL	NULL	0	NULL	cyclophilin-sensitive substrate	NULL	denatured	bind	NULL				GroEL	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_16_15_4568_s_9	9303301	(v) If a denatured cyclophilin-sensitive substrate is first bound to GroEL, however, productive folding to a cyclophilin-resistant form can be promoted, even without GroES.	bind
20354	2	5963	5	10	NULL	0	NULL	cyclophilin-sensitive substrate	NULL		folds to	NULL	productively			cyclophilin-resistant form	NULL				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_15_4568_s_9	9303301	(v) If a denatured cyclophilin-sensitive substrate is first bound to GroEL, however, productive folding to a cyclophilin-resistant form can be promoted, even without GroES.	bind
20355	3	5963	5	10	NULL	0	NULL	statement 2	NULL		occurs in absence of	NULL				GroES	NULL				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_15_4568_s_9	9303301	(v) If a denatured cyclophilin-sensitive substrate is first bound to GroEL, however, productive folding to a cyclophilin-resistant form can be promoted, even without GroES.	bind
45563	1	5963	7	NULL	NULL	NULL	NULL	cyclophilin-sensitive substrate	Chemical	denatured	bind					GroEL	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_15_4568_s_9	9303301	(v) If a denatured cyclophilin-sensitive substrate is first bound to GroEL, however, productive folding to a cyclophilin-resistant form can be promoted, even without GroES.	bind
45564	2	5963	7	NULL	NULL	NULL	NULL	cyclophilin-sensitive substrate	Chemical	denatured	 folds to		productively			 cyclophilin-resistant substrate	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_15_4568_s_9	9303301	(v) If a denatured cyclophilin-sensitive substrate is first bound to GroEL, however, productive folding to a cyclophilin-resistant form can be promoted, even without GroES.	bind
45565	3	5963	7	NULL	NULL	NULL	NULL	statement 2	Process		in the absence of					GroES	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_15_4568_s_9	9303301	(v) If a denatured cyclophilin-sensitive substrate is first bound to GroEL, however, productive folding to a cyclophilin-resistant form can be promoted, even without GroES.	bind
18468	1	5964	7	NULL	NULL	NULL	NULL	anti-Omp25	GP		bind					brucella	Organism				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_8_4823_s_231	11447156	(v) Macrophages infected with anti-Omp25-treated WT  B. suis produced TNF-alpha, an observation which is in line with a blockade of Omp25, since the anti-Omp25 antibody bound to an epitope of the protein which, in spite of LPS, was directly accessible on the bacteria and the comparison of the binding of anti-Omp25 and anti-Omp31 (two IgG2a MAbs) to  Brucella excluded the participation of the anti-Omp25 Fc group in TNF-alpha induction, as the levels of bound anti-Omp31 were significantly higher, yet the binding of anti-Omp31 exerted only a slight effect on the production of the cytokine during infection.	bind
18469	2	5964	7	NULL	NULL	NULL	NULL	anti-Omp31	GP		bind					brucella	Organism				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_8_4823_s_231	11447156	(v) Macrophages infected with anti-Omp25-treated WT  B. suis produced TNF-alpha, an observation which is in line with a blockade of Omp25, since the anti-Omp25 antibody bound to an epitope of the protein which, in spite of LPS, was directly accessible on the bacteria and the comparison of the binding of anti-Omp25 and anti-Omp31 (two IgG2a MAbs) to  Brucella excluded the participation of the anti-Omp25 Fc group in TNF-alpha induction, as the levels of bound anti-Omp31 were significantly higher, yet the binding of anti-Omp31 exerted only a slight effect on the production of the cytokine during infection.	bind
15467	1	5965	5	NULL	NULL	0	NULL	ATP	NULL		bind	NULL				TNFR1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_8_2536_s_209	11909948	(v) Mutations in the P-loop motif abolish ATP binding by TNFR1.	bind
15468	2	5965	5	NULL	NULL	0	NULL		NULL	mutant	abolish	NULL		P-loop motif		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_8_2536_s_209	11909948	(v) Mutations in the P-loop motif abolish ATP binding by TNFR1.	bind
18366	1	5965	7	NULL	NULL	NULL	NULL	ATP 	Chemical		bind					TNFR1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_8_2536_s_209	11909948	(v) Mutations in the P-loop motif abolish ATP binding by TNFR1.	bind
18367	2	5965	7	NULL	NULL	NULL	NULL			mutant	abolish			P-loop motif		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_8_2536_s_209	11909948	(v) Mutations in the P-loop motif abolish ATP binding by TNFR1.	bind
15469	1	5966	5	NULL	NULL	0	NULL	NF-kappaB proteins	NULL		bind	NULL				MMP-9	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_38_35766_s_10	12105194	(v) Recombinant IRF1, although unable to bind to an NF-kappaB consensus sequence, competes with NF-kappaB proteins for binding to the  MMP-9 promoter.	bind
15470	2	5966	5	NULL	NULL	0	NULL	IRF1	NULL	recombinant	does not bind	NULL					NULL			NF-kappaB consensus sequence	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_38_35766_s_10	12105194	(v) Recombinant IRF1, although unable to bind to an NF-kappaB consensus sequence, competes with NF-kappaB proteins for binding to the  MMP-9 promoter.	bind
15471	3	5966	5	NULL	NULL	0	NULL	IRF1	NULL	recombinant	bind	NULL				MMP-9	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_38_35766_s_10	12105194	(v) Recombinant IRF1, although unable to bind to an NF-kappaB consensus sequence, competes with NF-kappaB proteins for binding to the  MMP-9 promoter.	bind
15472	4	5966	5	NULL	NULL	0	NULL	statement 3	NULL		compete with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_38_35766_s_10	12105194	(v) Recombinant IRF1, although unable to bind to an NF-kappaB consensus sequence, competes with NF-kappaB proteins for binding to the  MMP-9 promoter.	bind
18368	1	5966	7	NULL	NULL	NULL	NULL	IRF1	GP	Recombinant	does not bind									NF-kappaB consensus sequence	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_38_35766_s_10	12105194	(v) Recombinant IRF1, although unable to bind to an NF-kappaB consensus sequence, competes with NF-kappaB proteins for binding to the  MMP-9 promoter.	bind
18369	2	5966	7	NULL	NULL	NULL	NULL	NF-kappaB protein	GP		binds					MMP-9	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_38_35766_s_10	12105194	(v) Recombinant IRF1, although unable to bind to an NF-kappaB consensus sequence, competes with NF-kappaB proteins for binding to the  MMP-9 promoter.	bind
18370	4	5966	7	NULL	NULL	NULL	NULL	statement 3	Process		compete with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_38_35766_s_10	12105194	(v) Recombinant IRF1, although unable to bind to an NF-kappaB consensus sequence, competes with NF-kappaB proteins for binding to the  MMP-9 promoter.	bind
25476	3	5966	7	NULL	NULL	NULL	NULL	IRF1	GP	recombinant	bind					MMP-9	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_38_35766_s_10	12105194	(v) Recombinant IRF1, although unable to bind to an NF-kappaB consensus sequence, competes with NF-kappaB proteins for binding to the  MMP-9 promoter.	bind
16324	1	5967	5	NULL	NULL	0	NULL	(V+C) FN	NULL		bind	NULL				PGs	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_13_11175_s_134	12482864	(V+C)  FN Binds Significantly More PGs Than Does V+C+ FN-- Analysis of small PG fractions bound to recombinant (V+C)  FN, recombinant V+C+ FN, and plasma FN revealed that the cartilage-specific isoform was able to bind small PGs despite the absence of protein segments V, III15, and I10 near the Hep II-binding domain.	bind
16325	2	5967	5	NULL	NULL	0	NULL	V+C+ FN	NULL		bind	NULL				PGs	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_13_11175_s_134	12482864	(V+C)  FN Binds Significantly More PGs Than Does V+C+ FN-- Analysis of small PG fractions bound to recombinant (V+C)  FN, recombinant V+C+ FN, and plasma FN revealed that the cartilage-specific isoform was able to bind small PGs despite the absence of protein segments V, III15, and I10 near the Hep II-binding domain.	bind
16326	3	5967	5	10	NULL	0	NULL	statement 1			more than		significantly			statement 2					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_13_11175_s_134	12482864	(V+C)  FN Binds Significantly More PGs Than Does V+C+ FN-- Analysis of small PG fractions bound to recombinant (V+C)  FN, recombinant V+C+ FN, and plasma FN revealed that the cartilage-specific isoform was able to bind small PGs despite the absence of protein segments V, III15, and I10 near the Hep II-binding domain.	bind
16328	4	5967	5	NULL	NULL	0	NULL	PG fractions	NULL	small	bind	NULL				(V+C) FN	NULL	recombinant			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_13_11175_s_134	12482864	(V+C)  FN Binds Significantly More PGs Than Does V+C+ FN-- Analysis of small PG fractions bound to recombinant (V+C)  FN, recombinant V+C+ FN, and plasma FN revealed that the cartilage-specific isoform was able to bind small PGs despite the absence of protein segments V, III15, and I10 near the Hep II-binding domain.	bind
16329	5	5967	5	NULL	NULL	0	NULL	PG fractions	NULL	small	bind	NULL				V+C+ FN	NULL	recombinant			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_13_11175_s_134	12482864	(V+C)  FN Binds Significantly More PGs Than Does V+C+ FN-- Analysis of small PG fractions bound to recombinant (V+C)  FN, recombinant V+C+ FN, and plasma FN revealed that the cartilage-specific isoform was able to bind small PGs despite the absence of protein segments V, III15, and I10 near the Hep II-binding domain.	bind
16330	6	5967	5	NULL	NULL	0	NULL	PG fractions	NULL	small	bind	NULL				FN	NULL	plasma			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_13_11175_s_134	12482864	(V+C)  FN Binds Significantly More PGs Than Does V+C+ FN-- Analysis of small PG fractions bound to recombinant (V+C)  FN, recombinant V+C+ FN, and plasma FN revealed that the cartilage-specific isoform was able to bind small PGs despite the absence of protein segments V, III15, and I10 near the Hep II-binding domain.	bind
16331	7	5967	5	NULL	NULL	0	NULL	cartilage-specific isoform	NULL		bind	NULL				PGs	NULL	small			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_13_11175_s_134	12482864	(V+C)  FN Binds Significantly More PGs Than Does V+C+ FN-- Analysis of small PG fractions bound to recombinant (V+C)  FN, recombinant V+C+ FN, and plasma FN revealed that the cartilage-specific isoform was able to bind small PGs despite the absence of protein segments V, III15, and I10 near the Hep II-binding domain.	bind
16332	8	5967	5	NULL	NULL	0	NULL	statement 7	NULL		occurs despite	NULL				protein segment V	NULL	absence of	near Hep II-binding domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_13_11175_s_134	12482864	(V+C)  FN Binds Significantly More PGs Than Does V+C+ FN-- Analysis of small PG fractions bound to recombinant (V+C)  FN, recombinant V+C+ FN, and plasma FN revealed that the cartilage-specific isoform was able to bind small PGs despite the absence of protein segments V, III15, and I10 near the Hep II-binding domain.	bind
16333	9	5967	5	NULL	NULL	0	NULL	statement 7	NULL		occurs despite	NULL				protein segment III15	NULL	absence of	near Hep II-binding domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_13_11175_s_134	12482864	(V+C)  FN Binds Significantly More PGs Than Does V+C+ FN-- Analysis of small PG fractions bound to recombinant (V+C)  FN, recombinant V+C+ FN, and plasma FN revealed that the cartilage-specific isoform was able to bind small PGs despite the absence of protein segments V, III15, and I10 near the Hep II-binding domain.	bind
16334	10	5967	5	NULL	NULL	0	NULL	statement 7	NULL		occurs despite	NULL				protein segment I10	NULL	absence of	near Hep II-binding domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_13_11175_s_134	12482864	(V+C)  FN Binds Significantly More PGs Than Does V+C+ FN-- Analysis of small PG fractions bound to recombinant (V+C)  FN, recombinant V+C+ FN, and plasma FN revealed that the cartilage-specific isoform was able to bind small PGs despite the absence of protein segments V, III15, and I10 near the Hep II-binding domain.	bind
18371	1	5967	7	NULL	NULL	NULL	NULL	(V+C) FN	GP		bind					PGs	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_13_11175_s_134	12482864	(V+C)  FN Binds Significantly More PGs Than Does V+C+ FN-- Analysis of small PG fractions bound to recombinant (V+C)  FN, recombinant V+C+ FN, and plasma FN revealed that the cartilage-specific isoform was able to bind small PGs despite the absence of protein segments V, III15, and I10 near the Hep II-binding domain.	bind
18372	2	5967	7	NULL	NULL	NULL	NULL	V+C+ FN	GP		bind					PGs	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_13_11175_s_134	12482864	(V+C)  FN Binds Significantly More PGs Than Does V+C+ FN-- Analysis of small PG fractions bound to recombinant (V+C)  FN, recombinant V+C+ FN, and plasma FN revealed that the cartilage-specific isoform was able to bind small PGs despite the absence of protein segments V, III15, and I10 near the Hep II-binding domain.	bind
18373	3	5967	7	NULL	NULL	NULL	NULL	statement 1	Process		more than		significantly			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_13_11175_s_134	12482864	(V+C)  FN Binds Significantly More PGs Than Does V+C+ FN-- Analysis of small PG fractions bound to recombinant (V+C)  FN, recombinant V+C+ FN, and plasma FN revealed that the cartilage-specific isoform was able to bind small PGs despite the absence of protein segments V, III15, and I10 near the Hep II-binding domain.	bind
18374	4	5967	7	NULL	NULL	NULL	NULL	PG	Chemical		bind					 FN	GP	plasma			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_13_11175_s_134	12482864	(V+C)  FN Binds Significantly More PGs Than Does V+C+ FN-- Analysis of small PG fractions bound to recombinant (V+C)  FN, recombinant V+C+ FN, and plasma FN revealed that the cartilage-specific isoform was able to bind small PGs despite the absence of protein segments V, III15, and I10 near the Hep II-binding domain.	bind
18375	5	5967	7	NULL	NULL	NULL	NULL	cartilage-specific isoform 	GP		bind					PGs	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_13_11175_s_134	12482864	(V+C)  FN Binds Significantly More PGs Than Does V+C+ FN-- Analysis of small PG fractions bound to recombinant (V+C)  FN, recombinant V+C+ FN, and plasma FN revealed that the cartilage-specific isoform was able to bind small PGs despite the absence of protein segments V, III15, and I10 near the Hep II-binding domain.	bind
18376	6	5967	7	NULL	NULL	NULL	NULL	statement 5	Process		occurs near								Hep II-binding domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_13_11175_s_134	12482864	(V+C)  FN Binds Significantly More PGs Than Does V+C+ FN-- Analysis of small PG fractions bound to recombinant (V+C)  FN, recombinant V+C+ FN, and plasma FN revealed that the cartilage-specific isoform was able to bind small PGs despite the absence of protein segments V, III15, and I10 near the Hep II-binding domain.	bind
18377	7	5967	7	NULL	NULL	NULL	NULL	statement 5	Process		occurs despite 					protein segment V	GP	absence of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_13_11175_s_134	12482864	(V+C)  FN Binds Significantly More PGs Than Does V+C+ FN-- Analysis of small PG fractions bound to recombinant (V+C)  FN, recombinant V+C+ FN, and plasma FN revealed that the cartilage-specific isoform was able to bind small PGs despite the absence of protein segments V, III15, and I10 near the Hep II-binding domain.	bind
18378	8	5967	7	NULL	NULL	NULL	NULL	statement 5	Process		occurs despite 					protein segment III15	GP	absence of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_13_11175_s_134	12482864	(V+C)  FN Binds Significantly More PGs Than Does V+C+ FN-- Analysis of small PG fractions bound to recombinant (V+C)  FN, recombinant V+C+ FN, and plasma FN revealed that the cartilage-specific isoform was able to bind small PGs despite the absence of protein segments V, III15, and I10 near the Hep II-binding domain.	bind
18379	9	5967	7	NULL	NULL	NULL	NULL	statement 5	Process		occurs despite					protein segment I10	GP	absence of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_13_11175_s_134	12482864	(V+C)  FN Binds Significantly More PGs Than Does V+C+ FN-- Analysis of small PG fractions bound to recombinant (V+C)  FN, recombinant V+C+ FN, and plasma FN revealed that the cartilage-specific isoform was able to bind small PGs despite the absence of protein segments V, III15, and I10 near the Hep II-binding domain.	bind
15617	1	5968	5	NULL	NULL	0	NULL	ITGA6/ITGB1	NULL		is	NULL				Epithelial 6 1 integrin	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_273_1_1_s_88	15302594	(vi) Epithelial  6 1 integrin (ITGA6/ITGB1)  and (vii) the long isoform of  1, (4-galactosyltransferaseB4GALT1) bind the laminin-1  (LAM1) G domain.	bind
15618	2	5968	5	NULL	NULL	0	NULL	ITGA6/ITGB1	NULL		bind	NULL				LAM1	NULL		G domain		NULL		0	NULL	NULL	NULL	gw70_devbiol_273_1_1_s_88	15302594	(vi) Epithelial  6 1 integrin (ITGA6/ITGB1)  and (vii) the long isoform of  1, (4-galactosyltransferaseB4GALT1) bind the laminin-1  (LAM1) G domain.	bind
15619	3	5968	5	NULL	NULL	0	NULL	LAM1	NULL		is	NULL				laminin-1	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_273_1_1_s_88	15302594	(vi) Epithelial  6 1 integrin (ITGA6/ITGB1)  and (vii) the long isoform of  1, (4-galactosyltransferaseB4GALT1) bind the laminin-1  (LAM1) G domain.	bind
15620	4	5968	5	NULL	NULL	0	NULL	long isoform of 1, (4-galactosyltransferaseB4GALT1)	NULL		bind	NULL				LAM1	NULL		G domain		NULL		0	NULL	NULL	NULL	gw70_devbiol_273_1_1_s_88	15302594	(vi) Epithelial  6 1 integrin (ITGA6/ITGB1)  and (vii) the long isoform of  1, (4-galactosyltransferaseB4GALT1) bind the laminin-1  (LAM1) G domain.	bind
18380	1	5968	7	NULL	NULL	NULL	NULL	Epithelial 6 1 integrin	GP		bind					laminin-1	GP		G domain		NULL		NULL	NULL	NULL	NULL	gw70_devbiol_273_1_1_s_88	15302594	(vi) Epithelial  6 1 integrin (ITGA6/ITGB1)  and (vii) the long isoform of  1, (4-galactosyltransferaseB4GALT1) bind the laminin-1  (LAM1) G domain.	bind
18381	2	5968	7	NULL	NULL	NULL	NULL	long isoform 1, (4-galactosyltransferaseB4GALT1)	GP		bind					laminin-1	GP		G domain		NULL		NULL	NULL	NULL	NULL	gw70_devbiol_273_1_1_s_88	15302594	(vi) Epithelial  6 1 integrin (ITGA6/ITGB1)  and (vii) the long isoform of  1, (4-galactosyltransferaseB4GALT1) bind the laminin-1  (LAM1) G domain.	bind
18382	3	5968	7	NULL	NULL	NULL	NULL	Epithelial 6 1 integrin	GP		is					ITGA6/ITGB1	GP				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_273_1_1_s_88	15302594	(vi) Epithelial  6 1 integrin (ITGA6/ITGB1)  and (vii) the long isoform of  1, (4-galactosyltransferaseB4GALT1) bind the laminin-1  (LAM1) G domain.	bind
18383	4	5968	7	NULL	NULL	NULL	NULL	LAM1	GP		is					 laminin-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_273_1_1_s_88	15302594	(vi) Epithelial  6 1 integrin (ITGA6/ITGB1)  and (vii) the long isoform of  1, (4-galactosyltransferaseB4GALT1) bind the laminin-1  (LAM1) G domain.	bind
15621	1	5969	5	NULL	NULL	0	NULL	Fibrinogen	NULL		bind	NULL				platelet alpha(IIb)beta3 receptor	NULL				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_j-thromb-haemost_3_8_16102057_s_17	16102057	(vi) Fibrinogen  binding to the platelet alpha(IIb)beta3 receptor, which is important for  incorporating platelets into a developing thrombus.	bind
15622	2	5969	5	NULL	NULL	0	NULL	statement 1	NULL		is important for	NULL				developing thrombus	NULL	incorporating platelets into			NULL		0	NULL	NULL	NULL	abs-batch0530-0539_j-thromb-haemost_3_8_16102057_s_17	16102057	(vi) Fibrinogen  binding to the platelet alpha(IIb)beta3 receptor, which is important for  incorporating platelets into a developing thrombus.	bind
18385	1	5969	7	NULL	NULL	NULL	NULL	Fibrinogen	GP		bind					platelet alpha(IIb)beta3 receptor	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_j-thromb-haemost_3_8_16102057_s_17	16102057	(vi) Fibrinogen  binding to the platelet alpha(IIb)beta3 receptor, which is important for  incorporating platelets into a developing thrombus.	bind
18386	2	5969	7	NULL	NULL	NULL	NULL	statement 1	Process		is important for					developing thrombus	Process	 incorporating platelets into a			NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_j-thromb-haemost_3_8_16102057_s_17	16102057	(vi) Fibrinogen  binding to the platelet alpha(IIb)beta3 receptor, which is important for  incorporating platelets into a developing thrombus.	bind
15623	1	5970	5	NULL	NULL	0	NULL	GerK	NULL		bind	NULL				glucose	NULL				NULL		0	NULL	NULL	NULL	abs-batch0600-0619_j-bacteriol_188_1_16352818_s_14	16352818	(vi) GerK binds glucose, GerB interacts  with fructose in addition to L-amino acids, and GerA interacts only with  L-valine, L-alanine, and its analogs.	bind
15624	2	5970	5	NULL	NULL	0	NULL	GerB	NULL		interacts with	NULL				fructose	NULL				NULL		0	NULL	NULL	NULL	abs-batch0600-0619_j-bacteriol_188_1_16352818_s_14	16352818	(vi) GerK binds glucose, GerB interacts  with fructose in addition to L-amino acids, and GerA interacts only with  L-valine, L-alanine, and its analogs.	bind
15625	3	5970	5	NULL	NULL	0	NULL	GerB	NULL		interacts with	NULL				L-amino acids	NULL				NULL		0	NULL	NULL	NULL	abs-batch0600-0619_j-bacteriol_188_1_16352818_s_14	16352818	(vi) GerK binds glucose, GerB interacts  with fructose in addition to L-amino acids, and GerA interacts only with  L-valine, L-alanine, and its analogs.	bind
15626	4	5970	5	NULL	NULL	0	NULL	GerA	NULL		interacts with	NULL				L-valine	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_j-bacteriol_188_1_16352818_s_14	16352818	(vi) GerK binds glucose, GerB interacts  with fructose in addition to L-amino acids, and GerA interacts only with  L-valine, L-alanine, and its analogs.	bind
15627	5	5970	5	NULL	NULL	0	NULL	GerA	NULL		interacts with	NULL				L-alanine	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_j-bacteriol_188_1_16352818_s_14	16352818	(vi) GerK binds glucose, GerB interacts  with fructose in addition to L-amino acids, and GerA interacts only with  L-valine, L-alanine, and its analogs.	bind
15628	6	5970	5	NULL	NULL	0	NULL	GerA	NULL		interacts with	NULL				L-alanine	NULL	analogs of			NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_j-bacteriol_188_1_16352818_s_14	16352818	(vi) GerK binds glucose, GerB interacts  with fructose in addition to L-amino acids, and GerA interacts only with  L-valine, L-alanine, and its analogs.	bind
15629	7	5970	5	NULL	NULL	0	NULL	GerA	NULL		interacts with	NULL				L-valine	NULL	analogs of			NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_j-bacteriol_188_1_16352818_s_14	16352818	(vi) GerK binds glucose, GerB interacts  with fructose in addition to L-amino acids, and GerA interacts only with  L-valine, L-alanine, and its analogs.	bind
18387	1	5970	7	NULL	NULL	NULL	NULL	GerK	GP		binds					glucose	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_j-bacteriol_188_1_16352818_s_14	16352818	(vi) GerK binds glucose, GerB interacts  with fructose in addition to L-amino acids, and GerA interacts only with  L-valine, L-alanine, and its analogs.	bind
18388	2	5970	7	NULL	NULL	NULL	NULL	GerB	GP		interacts with					fructose	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_j-bacteriol_188_1_16352818_s_14	16352818	(vi) GerK binds glucose, GerB interacts  with fructose in addition to L-amino acids, and GerA interacts only with  L-valine, L-alanine, and its analogs.	bind
18389	3	5970	7	NULL	NULL	NULL	NULL	GerB	GP		interacts with					L-amino acids	AminoAcid				NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_j-bacteriol_188_1_16352818_s_14	16352818	(vi) GerK binds glucose, GerB interacts  with fructose in addition to L-amino acids, and GerA interacts only with  L-valine, L-alanine, and its analogs.	bind
18390	4	5970	7	NULL	NULL	NULL	NULL	GerA	GP		interacts with					L-valine	AminoAcid				NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_j-bacteriol_188_1_16352818_s_14	16352818	(vi) GerK binds glucose, GerB interacts  with fructose in addition to L-amino acids, and GerA interacts only with  L-valine, L-alanine, and its analogs.	bind
18391	5	5970	7	NULL	NULL	NULL	NULL	GerA	GP		interacts with					L-alanine	AminoAcid				NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_j-bacteriol_188_1_16352818_s_14	16352818	(vi) GerK binds glucose, GerB interacts  with fructose in addition to L-amino acids, and GerA interacts only with  L-valine, L-alanine, and its analogs.	bind
18392	6	5970	7	NULL	NULL	NULL	NULL	GerA	GP		interacts with					L-valine	AminoAcid	analogs of			NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_j-bacteriol_188_1_16352818_s_14	16352818	(vi) GerK binds glucose, GerB interacts  with fructose in addition to L-amino acids, and GerA interacts only with  L-valine, L-alanine, and its analogs.	bind
18393	7	5970	7	NULL	NULL	NULL	NULL	GerA	GP		interacts with					L-alanine	AminoAcid	analogs of			NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_j-bacteriol_188_1_16352818_s_14	16352818	(vi) GerK binds glucose, GerB interacts  with fructose in addition to L-amino acids, and GerA interacts only with  L-valine, L-alanine, and its analogs.	bind
15630	1	5973	5	NULL	NULL	0	NULL	IGF-I	NULL		mediate	NULL				IGF-IR	NULL	ubiquitination of			NULL	p6 cells	0	NULL	NULL	NULL	gw60_molcellbiol_23_9_3363_s_270	12697834	(vii) Overexpression of a Grb10 mutant lacking the SH2 domain impairs IGF-I-mediated ubiquitination of the IGF-IR in both p6 and p6/Grb10 cells, suggesting that binding between Grb10 and Nedd4 is critical for ubiquitination of the receptor.	bind
15631	2	5973	5	NULL	NULL	0	NULL	IGF-I	NULL		mediate	NULL				IGF-IR	NULL	ubiquitination of			NULL	p6/Grb10 cells	0	NULL	NULL	NULL	gw60_molcellbiol_23_9_3363_s_270	12697834	(vii) Overexpression of a Grb10 mutant lacking the SH2 domain impairs IGF-I-mediated ubiquitination of the IGF-IR in both p6 and p6/Grb10 cells, suggesting that binding between Grb10 and Nedd4 is critical for ubiquitination of the receptor.	bind
15632	3	5973	5	10	NULL	0	NULL	Grb10	NULL	overexpression of;; mutant	impairs	NULL		SH2 domain		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_9_3363_s_270	12697834	(vii) Overexpression of a Grb10 mutant lacking the SH2 domain impairs IGF-I-mediated ubiquitination of the IGF-IR in both p6 and p6/Grb10 cells, suggesting that binding between Grb10 and Nedd4 is critical for ubiquitination of the receptor.	bind
15633	4	5973	5	10	NULL	0	NULL	Grb10	NULL	overexpression of;; mutant 	impairs	NULL		SH2 domain		statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_9_3363_s_270	12697834	(vii) Overexpression of a Grb10 mutant lacking the SH2 domain impairs IGF-I-mediated ubiquitination of the IGF-IR in both p6 and p6/Grb10 cells, suggesting that binding between Grb10 and Nedd4 is critical for ubiquitination of the receptor.	bind
15634	5	5973	5	NULL	NULL	0	NULL	Grb10	NULL		bind	NULL				Nedd4	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_9_3363_s_270	12697834	(vii) Overexpression of a Grb10 mutant lacking the SH2 domain impairs IGF-I-mediated ubiquitination of the IGF-IR in both p6 and p6/Grb10 cells, suggesting that binding between Grb10 and Nedd4 is critical for ubiquitination of the receptor.	bind
15635	6	5973	5	NULL	NULL	0	NULL	statement 5	NULL		critical for	NULL				IGF-IR	NULL	ubiquitination of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_9_3363_s_270	12697834	(vii) Overexpression of a Grb10 mutant lacking the SH2 domain impairs IGF-I-mediated ubiquitination of the IGF-IR in both p6 and p6/Grb10 cells, suggesting that binding between Grb10 and Nedd4 is critical for ubiquitination of the receptor.	bind
15636	7	5973	5	NULL	NULL	0	NULL	statement 3	NULL		suggest	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_9_3363_s_270	12697834	(vii) Overexpression of a Grb10 mutant lacking the SH2 domain impairs IGF-I-mediated ubiquitination of the IGF-IR in both p6 and p6/Grb10 cells, suggesting that binding between Grb10 and Nedd4 is critical for ubiquitination of the receptor.	bind
15637	8	5973	5	NULL	NULL	0	NULL	statement 4	NULL		suggest	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_9_3363_s_270	12697834	(vii) Overexpression of a Grb10 mutant lacking the SH2 domain impairs IGF-I-mediated ubiquitination of the IGF-IR in both p6 and p6/Grb10 cells, suggesting that binding between Grb10 and Nedd4 is critical for ubiquitination of the receptor.	bind
18394	1	5973	7	NULL	NULL	NULL	NULL	IGF-I	GP		mediates					IGF-IR	GP	 ubiquitination of			NULL	p6 cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_23_9_3363_s_270	12697834	(vii) Overexpression of a Grb10 mutant lacking the SH2 domain impairs IGF-I-mediated ubiquitination of the IGF-IR in both p6 and p6/Grb10 cells, suggesting that binding between Grb10 and Nedd4 is critical for ubiquitination of the receptor.	bind
18395	2	5973	7	NULL	NULL	NULL	NULL	IGF-I	GP		mediates					IGF-IR	GP	ubiquitination of			NULL	p6/Grb10 cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_23_9_3363_s_270	12697834	(vii) Overexpression of a Grb10 mutant lacking the SH2 domain impairs IGF-I-mediated ubiquitination of the IGF-IR in both p6 and p6/Grb10 cells, suggesting that binding between Grb10 and Nedd4 is critical for ubiquitination of the receptor.	bind
18396	3	5973	7	NULL	NULL	NULL	NULL	Grb10	GP	overexpression of;; mutant	impairs			SH2 domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_9_3363_s_270	12697834	(vii) Overexpression of a Grb10 mutant lacking the SH2 domain impairs IGF-I-mediated ubiquitination of the IGF-IR in both p6 and p6/Grb10 cells, suggesting that binding between Grb10 and Nedd4 is critical for ubiquitination of the receptor.	bind
18397	4	5973	7	NULL	NULL	NULL	NULL	Grb10	GP	overexpression of;; mutant	impairs			SH2 domain		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_9_3363_s_270	12697834	(vii) Overexpression of a Grb10 mutant lacking the SH2 domain impairs IGF-I-mediated ubiquitination of the IGF-IR in both p6 and p6/Grb10 cells, suggesting that binding between Grb10 and Nedd4 is critical for ubiquitination of the receptor.	bind
18398	5	5973	7	NULL	NULL	NULL	NULL	Grb10	GP		bind					Nedd4	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_9_3363_s_270	12697834	(vii) Overexpression of a Grb10 mutant lacking the SH2 domain impairs IGF-I-mediated ubiquitination of the IGF-IR in both p6 and p6/Grb10 cells, suggesting that binding between Grb10 and Nedd4 is critical for ubiquitination of the receptor.	bind
18399	6	5973	7	NULL	NULL	NULL	NULL	statement 5	Process		is critical for					IGF-IR	GP	ubiquitination of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_9_3363_s_270	12697834	(vii) Overexpression of a Grb10 mutant lacking the SH2 domain impairs IGF-I-mediated ubiquitination of the IGF-IR in both p6 and p6/Grb10 cells, suggesting that binding between Grb10 and Nedd4 is critical for ubiquitination of the receptor.	bind
15638	1	5974	5	NULL	NULL	0	NULL	vWF	NULL		bind	NULL				collagen type I	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_91_5_1354_s_26	7867173	(vWF can bind to collagen types I, II, and VI. 9 10  Collagen type I predominates in atherosclerotic arterial subendothelium.	bind
15639	2	5974	5	NULL	NULL	0	NULL	vWF	NULL		bind	NULL				collagen type II	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_91_5_1354_s_26	7867173	(vWF can bind to collagen types I, II, and VI. 9 10  Collagen type I predominates in atherosclerotic arterial subendothelium.	bind
15640	3	5974	5	NULL	NULL	0	NULL	vWF	NULL		bind	NULL				collagen type VI	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_91_5_1354_s_26	7867173	(vWF can bind to collagen types I, II, and VI. 9 10  Collagen type I predominates in atherosclerotic arterial subendothelium.	bind
15641	4	5974	5	NULL	NULL	0	NULL	Collagen type I	NULL		predominates in	NULL				atherosclerotic arterial subendothelium	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_91_5_1354_s_26	7867173	(vWF can bind to collagen types I, II, and VI. 9 10  Collagen type I predominates in atherosclerotic arterial subendothelium.	bind
18400	1	5974	7	NULL	NULL	NULL	NULL	vWF	GP		bind					collagen type I	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1354_s_26	7867173	(vWF can bind to collagen types I, II, and VI. 9 10  Collagen type I predominates in atherosclerotic arterial subendothelium.	bind
18401	2	5974	7	NULL	NULL	NULL	NULL	vWF	GP		bind					collagen type II	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1354_s_26	7867173	(vWF can bind to collagen types I, II, and VI. 9 10  Collagen type I predominates in atherosclerotic arterial subendothelium.	bind
18402	3	5974	7	NULL	NULL	NULL	NULL	vWF	GP		bind					collagen type VI	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1354_s_26	7867173	(vWF can bind to collagen types I, II, and VI. 9 10  Collagen type I predominates in atherosclerotic arterial subendothelium.	bind
18403	4	5974	7	NULL	NULL	NULL	NULL	collagen type I	GP		predominates in					atherosclerotic arterial subendothelium	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1354_s_26	7867173	(vWF can bind to collagen types I, II, and VI. 9 10  Collagen type I predominates in atherosclerotic arterial subendothelium.	bind
15642	1	5976	5	NULL	NULL	0	NULL	MR	NULL		bind	NULL				cortisol	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_107_19_2512_s_26	12756192	(While the MR binds cortisol with equal affinity, tissue specificity for aldosterone is conferred by the local expression of the enzyme 11beta-hydroxysteroid dehydrogenase (11betaHSD) type 2, which converts cortisol and corticosterone into the inactive cortisone and 11-dehydrocorticosterone.	bind
15643	2	5976	5	NULL	NULL	0	NULL	(11betaHSD) type 2	NULL		is	NULL				enzyme 11beta-hydroxysteroid dehydrogenase type 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_19_2512_s_26	12756192	(While the MR binds cortisol with equal affinity, tissue specificity for aldosterone is conferred by the local expression of the enzyme 11beta-hydroxysteroid dehydrogenase (11betaHSD) type 2, which converts cortisol and corticosterone into the inactive cortisone and 11-dehydrocorticosterone.	bind
15644	3	5976	5	NULL	NULL	0	NULL	cortisol	NULL		is converted to	NULL				cortisone	NULL	inactive 			NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_19_2512_s_26	12756192	(While the MR binds cortisol with equal affinity, tissue specificity for aldosterone is conferred by the local expression of the enzyme 11beta-hydroxysteroid dehydrogenase (11betaHSD) type 2, which converts cortisol and corticosterone into the inactive cortisone and 11-dehydrocorticosterone.	bind
15645	4	5976	5	NULL	NULL	0	NULL	(11betaHSD) type 2	NULL		is required for	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_107_19_2512_s_26	12756192	(While the MR binds cortisol with equal affinity, tissue specificity for aldosterone is conferred by the local expression of the enzyme 11beta-hydroxysteroid dehydrogenase (11betaHSD) type 2, which converts cortisol and corticosterone into the inactive cortisone and 11-dehydrocorticosterone.	bind
15646	5	5976	5	NULL	NULL	0	NULL	corticosterone	NULL		is converted to	NULL				11-dehydrocorticosterone	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_107_19_2512_s_26	12756192	(While the MR binds cortisol with equal affinity, tissue specificity for aldosterone is conferred by the local expression of the enzyme 11beta-hydroxysteroid dehydrogenase (11betaHSD) type 2, which converts cortisol and corticosterone into the inactive cortisone and 11-dehydrocorticosterone.	bind
15647	6	5976	5	NULL	NULL	0	NULL	(11betaHSD) type 2	NULL		is required for	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_107_19_2512_s_26	12756192	(While the MR binds cortisol with equal affinity, tissue specificity for aldosterone is conferred by the local expression of the enzyme 11beta-hydroxysteroid dehydrogenase (11betaHSD) type 2, which converts cortisol and corticosterone into the inactive cortisone and 11-dehydrocorticosterone.	bind
20356	7	5976	5	NULL	NULL	0	NULL	aldosterone	NULL	tissue specificity for	is conferred by	NULL				(11betaHSD) type 2	NULL	 local expression of			NULL		0	NULL	NULL	NULL	gw70_circulation_107_19_2512_s_26	12756192	(While the MR binds cortisol with equal affinity, tissue specificity for aldosterone is conferred by the local expression of the enzyme 11beta-hydroxysteroid dehydrogenase (11betaHSD) type 2, which converts cortisol and corticosterone into the inactive cortisone and 11-dehydrocorticosterone.	bind
18404	1	5976	7	NULL	NULL	NULL	NULL	MR	GP		binds					cortisol	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_19_2512_s_26	12756192	(While the MR binds cortisol with equal affinity, tissue specificity for aldosterone is conferred by the local expression of the enzyme 11beta-hydroxysteroid dehydrogenase (11betaHSD) type 2, which converts cortisol and corticosterone into the inactive cortisone and 11-dehydrocorticosterone.	bind
18405	2	5976	7	NULL	NULL	NULL	NULL	cortisol	Chemical		is converted to					cortisone	Chemical	inactive			NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_19_2512_s_26	12756192	(While the MR binds cortisol with equal affinity, tissue specificity for aldosterone is conferred by the local expression of the enzyme 11beta-hydroxysteroid dehydrogenase (11betaHSD) type 2, which converts cortisol and corticosterone into the inactive cortisone and 11-dehydrocorticosterone.	bind
18406	3	5976	7	NULL	NULL	NULL	NULL	corticosterone	Chemical		is converted to					11-dehydrocorticosterone	Chemical	inactive			NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_19_2512_s_26	12756192	(While the MR binds cortisol with equal affinity, tissue specificity for aldosterone is conferred by the local expression of the enzyme 11beta-hydroxysteroid dehydrogenase (11betaHSD) type 2, which converts cortisol and corticosterone into the inactive cortisone and 11-dehydrocorticosterone.	bind
18407	4	5976	7	NULL	NULL	NULL	NULL	statement 2	Process		is carried out by					11betaHSD type 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_19_2512_s_26	12756192	(While the MR binds cortisol with equal affinity, tissue specificity for aldosterone is conferred by the local expression of the enzyme 11beta-hydroxysteroid dehydrogenase (11betaHSD) type 2, which converts cortisol and corticosterone into the inactive cortisone and 11-dehydrocorticosterone.	bind
18408	5	5976	7	NULL	NULL	NULL	NULL	statement 3	Process		is carried out by					11betaHSD type 2	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_19_2512_s_26	12756192	(While the MR binds cortisol with equal affinity, tissue specificity for aldosterone is conferred by the local expression of the enzyme 11beta-hydroxysteroid dehydrogenase (11betaHSD) type 2, which converts cortisol and corticosterone into the inactive cortisone and 11-dehydrocorticosterone.	bind
18409	6	5976	7	NULL	NULL	NULL	NULL	aldosterone	Chemical	tissue specificity for	is conferred by					11betaHSD type 2	Chemical	local expression of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_19_2512_s_26	12756192	(While the MR binds cortisol with equal affinity, tissue specificity for aldosterone is conferred by the local expression of the enzyme 11beta-hydroxysteroid dehydrogenase (11betaHSD) type 2, which converts cortisol and corticosterone into the inactive cortisone and 11-dehydrocorticosterone.	bind
18410	7	5976	7	NULL	NULL	NULL	NULL	11betaHSD	Chemical		is					11beta-hydroxysteroid dehydrogenase	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_19_2512_s_26	12756192	(While the MR binds cortisol with equal affinity, tissue specificity for aldosterone is conferred by the local expression of the enzyme 11beta-hydroxysteroid dehydrogenase (11betaHSD) type 2, which converts cortisol and corticosterone into the inactive cortisone and 11-dehydrocorticosterone.	bind
15648	1	5977	5	10	NULL	0	NULL	Verprolin-homologous protein			is an effector of		downstream			IRSp53					NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-neurosci_25_4_15673667_s_10	15673667	(Wiskott-Aldrich  syndrome protein family Verprolin-homologous protein), a downstream effector  of IRSp53 that binds to the SH3 domain of IRSp53.	bind
15649	2	5977	5	NULL	NULL	0	NULL	Verprolin-homologous protein	NULL		bind	NULL				IRSp53	NULL		SH3 domain		NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-neurosci_25_4_15673667_s_10	15673667	(Wiskott-Aldrich  syndrome protein family Verprolin-homologous protein), a downstream effector  of IRSp53 that binds to the SH3 domain of IRSp53.	bind
44809	3	5977	5	10	NULL	0	NULL	Verprolin-homologous protein	NULL		belongs to 	NULL				Wiskott-Aldrich syndrome protein family	NULL				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_j-neurosci_25_4_15673667_s_10	15673667	(Wiskott-Aldrich  syndrome protein family Verprolin-homologous protein), a downstream effector  of IRSp53 that binds to the SH3 domain of IRSp53.	bind
18420	1	5977	7	NULL	NULL	NULL	NULL	Verprolin-homologous protein	GP		binds					IRSp53	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-neurosci_25_4_15673667_s_10	15673667	(Wiskott-Aldrich  syndrome protein family Verprolin-homologous protein), a downstream effector  of IRSp53 that binds to the SH3 domain of IRSp53.	bind
18421	2	5977	7	NULL	NULL	NULL	NULL	Verprolin-homologous protein	GP		belongs to					Wiskott-Aldrich syndrome protein family	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-neurosci_25_4_15673667_s_10	15673667	(Wiskott-Aldrich  syndrome protein family Verprolin-homologous protein), a downstream effector  of IRSp53 that binds to the SH3 domain of IRSp53.	bind
18422	3	5977	7	NULL	NULL	NULL	NULL	Verprolin-homologous protein	GP		is an effector of		downstream			IRSp53	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-neurosci_25_4_15673667_s_10	15673667	(Wiskott-Aldrich  syndrome protein family Verprolin-homologous protein), a downstream effector  of IRSp53 that binds to the SH3 domain of IRSp53.	bind
15650	1	5982	5	NULL	NULL	0	NULL	iso-1 cytochrome c	NULL	yeast	bind	NULL				heme lyase	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_40_25695_s_198	9748237	([I]), gave the dissociation constant ( K i) for the binding of yeast iso-1 cytochrome  c to heme lyase	bind
18424	1	5982	7	NULL	NULL	NULL	NULL	iso-1 cytochrome c	GP	yeast	bind					heme lyase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_40_25695_s_198	9748237	([I]), gave the dissociation constant ( K i) for the binding of yeast iso-1 cytochrome  c to heme lyase	bind
15651	1	5984	5	NULL	NULL	0	NULL	NGF	NULL		induce	NULL				ERK	NULL	phosphorylation			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_6_1931_s_145	10688641	+ Ca2 chelatorsblock NGF-induced ERK phosphorylation.	bind
15652	2	5984	5	NULL	NULL	0	NULL	Ca2+ chelators	NULL		block	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_6_1931_s_145	10688641	+ Ca2 chelatorsblock NGF-induced ERK phosphorylation.	bind
18425	1	5984	7	NULL	NULL	NULL	NULL	NGF	GP		induce					ERK	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_1931_s_145	10688641	+ Ca2 chelatorsblock NGF-induced ERK phosphorylation.	bind
18426	2	5984	7	NULL	NULL	NULL	NULL	Ca2 chelators	Chemical		block					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_1931_s_145	10688641	+ Ca2 chelatorsblock NGF-induced ERK phosphorylation.	bind
15653	1	5986	5	NULL	NULL	0	NULL	DPPIV	NULL		bind	NULL				MBP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_27_24600_s_121	12716896	,   p <  0.01, relative to DPPIV binding to MBP.	bind
18428	1	5986	7	NULL	NULL	NULL	NULL	DPPIV	GP		bind					MBP	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_27_24600_s_121	12716896	,   p <  0.01, relative to DPPIV binding to MBP.	bind
15654	1	5988	5	NULL	NULL	0	NULL	spliceosomal 15.5 kD protein	NULL		bind	NULL				U4 snRNA fragment	NULL				NULL		NULL	NULL	NULL	NULL	gw70_nature_441_7097_1172_s_157	16810258	,  Nottrott, S. ,  Hartmuth, K. ,  Luhrmann, [[ R.  &  Ficner ]], R.   Crystal structure of the spliceosomal 15.5 kD protein bound to a U4 snRNA fragment.	bind
18500	1	5988	7	NULL	NULL	NULL	NULL	spliceosomal 15.5 kD protein	GP		bind					U4 snRNA fragment	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_nature_441_7097_1172_s_157	16810258	,  Nottrott, S. ,  Hartmuth, K. ,  Luhrmann, [[ R.  &  Ficner ]], R.   Crystal structure of the spliceosomal 15.5 kD protein bound to a U4 snRNA fragment.	bind
15655	1	5989	5	NULL	NULL	0	NULL	DPPIV	NULL		bind	NULL				MBP-FNIII12	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_27_24600_s_164	12716896	,  p < 0.01, relative to DPPIV binding to MBP-FNIII12  ( B) and relative to MTF7 adhesion to DPPIV-coated dishes  ( C).	bind
15656	2	5989	5	NULL	NULL	0	NULL	MTF7	NULL		adhere to	NULL				DPPIV	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_27_24600_s_164	12716896	,  p < 0.01, relative to DPPIV binding to MBP-FNIII12  ( B) and relative to MTF7 adhesion to DPPIV-coated dishes  ( C).	bind
18501	1	5989	7	NULL	NULL	NULL	NULL	DPPIV	GP		bind					MBP-FNIII12	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_27_24600_s_164	12716896	,  p < 0.01, relative to DPPIV binding to MBP-FNIII12  ( B) and relative to MTF7 adhesion to DPPIV-coated dishes  ( C).	bind
18502	2	5989	7	NULL	NULL	NULL	NULL	MTF7	GP		adhesion to					DPPIV-coated dishes	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_27_24600_s_164	12716896	,  p < 0.01, relative to DPPIV binding to MBP-FNIII12  ( B) and relative to MTF7 adhesion to DPPIV-coated dishes  ( C).	bind
15657	1	5992	5	NULL	NULL	0	NULL	NMDA antagonists	NULL		bind	NULL					NULL		glycine site		NULL		0	NULL	NULL	NULL	gw60_neurobioldis_12_1_82_s_8	12609492	, 1997) and noncompetitive NMDA receptor antagonists  ( Albers et al 1995 and   Lees 1997), as well as NMDA antagonists binding the glycine site  ( et al et al 2000 and   Sacco et al 2001), showed marked side effects and scant clinical efficacy.	bind
54138	2	5992	5	10	NULL	0	NULL	NMDA receptor antagonists		noncompetitive	bind								glycine site		NULL		0	NULL	NULL	NULL	gw60_neurobioldis_12_1_82_s_8	12609492	, 1997) and noncompetitive NMDA receptor antagonists  ( Albers et al 1995 and   Lees 1997), as well as NMDA antagonists binding the glycine site  ( et al et al 2000 and   Sacco et al 2001), showed marked side effects and scant clinical efficacy.	bind
18505	1	5992	7	NULL	NULL	NULL	NULL	NMDA receptor antagonists 	GP	noncompetitive	bind								glycine site		NULL		NULL	NULL	NULL	NULL	gw60_neurobioldis_12_1_82_s_8	12609492	, 1997) and noncompetitive NMDA receptor antagonists  ( Albers et al 1995 and   Lees 1997), as well as NMDA antagonists binding the glycine site  ( et al et al 2000 and   Sacco et al 2001), showed marked side effects and scant clinical efficacy.	bind
18506	2	5992	7	NULL	NULL	NULL	NULL	NMDA antagonists	GP		bind								glycine site		NULL		NULL	NULL	NULL	NULL	gw60_neurobioldis_12_1_82_s_8	12609492	, 1997) and noncompetitive NMDA receptor antagonists  ( Albers et al 1995 and   Lees 1997), as well as NMDA antagonists binding the glycine site  ( et al et al 2000 and   Sacco et al 2001), showed marked side effects and scant clinical efficacy.	bind
15658	1	5993	5	NULL	NULL	0	NULL	Wnt 	NULL		bind	NULL			response elements	Tcf-3	NULL				NULL		0	NULL	NULL	NULL	gw60_devbiol_257_1_190_s_350	12710967	, 1997) and the Wnt response elements bound by Tcf-3  ( Brannon et al 1997;  Laurent et al 1997 and   McKendry et al 1997).	bind
18507	1	5993	7	NULL	NULL	NULL	NULL	Tcf-3	GP		bind					 Wnt	GP			response element	NULL		NULL	NULL	NULL	NULL	gw60_devbiol_257_1_190_s_350	12710967	, 1997) and the Wnt response elements bound by Tcf-3  ( Brannon et al 1997;  Laurent et al 1997 and   McKendry et al 1997).	bind
15659	1	5995	5	NULL	NULL	0	NULL	MDM2	NULL		bind	NULL				pRb	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_25_22615_s_107	12702724	, binding between MDM2 and pRb or Sp1  was  determined previously ( ).	bind
15660	2	5995	5	NULL	NULL	0	NULL	MDM2	NULL		bind	NULL				Sp1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_25_22615_s_107	12702724	, binding between MDM2 and pRb or Sp1  was  determined previously ( ).	bind
15661	3	5995	5	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_25_22615_s_107	12702724	, binding between MDM2 and pRb or Sp1  was  determined previously ( ).	bind
18508	1	5995	7	NULL	NULL	NULL	NULL	MDM2	GP		bind					pRb	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_25_22615_s_107	12702724	, binding between MDM2 and pRb or Sp1  was  determined previously ( ).	bind
18509	2	5995	7	NULL	NULL	NULL	NULL	MDM2	GP		bind					Sp1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_25_22615_s_107	12702724	, binding between MDM2 and pRb or Sp1  was  determined previously ( ).	bind
18510	3	5995	7	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_25_22615_s_107	12702724	, binding between MDM2 and pRb or Sp1  was  determined previously ( ).	bind
15663	1	5997	5	NULL	NULL	0	NULL	calpain	NULL	inactive native	associate with	NULL	reversibly			plasma membrane	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
15664	2	5997	5	NULL	NULL	0	NULL	Ca2+	NULL		induce	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
15666	3	5997	5	NULL	NULL	0	NULL	conformational changes	NULL	low Ca2+-induced	produce	NULL				calpain	NULL	active native			NULL	onto the inner surface of the plasma membrane	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
15667	4	5997	5	NULL	NULL	0	NULL	calpain	NULL	active	undergoes	NULL				autoproteolysis	NULL	irreversible			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
15668	5	5997	5	NULL	NULL	0	NULL	conformational changes	NULL	high Ca2+-induced	produce	NULL				calpain	NULL	soluble active native			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
15669	6	5997	5	NULL	NULL	0	NULL	calpain	NULL	soluble active	associate with	NULL	possibly			plasma membrane	NULL	inner surface of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
15670	7	5997	5	NULL	NULL	0	NULL	calpain	NULL	autoproteolyzed active	is released from	NULL	spontaneously			plasma membrane	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
15671	8	5997	5	NULL	NULL	0	NULL	calpain	NULL	active native	undergoes	NULL	possibly			autoproteolysis	NULL				NULL	in cytosol	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
15672	9	5997	5	NULL	NULL	0	NULL	statement 8	NULL		requires	NULL				Ca2+	NULL	high			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
15673	10	5997	5	NULL	NULL	0	NULL	calpastatin	NULL		bind	NULL	high affinity			calpain	NULL	autoproteolyzed			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
15674	11	5997	5	NULL	NULL	0	NULL	statement 10	NULL		inhibit	NULL				calpain	NULL	catalytic activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
15675	12	5997	5	NULL	NULL	0	NULL	calpastatin	NULL		is degraded to	NULL				fragments	NULL	active			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
15676	13	5997	5	NULL	NULL	0	NULL	calpastatin	NULL		is degraded to	NULL				fragments	NULL	inactive			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
15677	14	5997	5	NULL	NULL	0	NULL	calpastatin	NULL		bind	NULL				calpain	NULL	active native			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
15678	15	5997	5	NULL	NULL	0	NULL	statement 14	NULL		inhibit	NULL				calpain	NULL	catalytic activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
15679	16	5997	5	NULL	NULL	0	NULL	calpastatin	NULL		is degraded to	NULL				fragments	NULL	active, at lower rate			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
15680	17	5997	5	NULL	NULL	0	NULL	calpastatin	NULL		is degraded to	NULL				fragments	NULL	inactive, at lower rate			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
18829	1	5997	7	NULL	NULL	NULL	NULL	calpain 	GP	inactive native	binds					plasma membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
18830	2	5997	7	NULL	NULL	NULL	NULL	Ca2+	Chemical		induce					statement 1	Process	reversible association of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
18831	3	5997	7	NULL	NULL	NULL	NULL	calpain	GP	active native	on					plasma membrane	CellComponent	inner surface of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
18832	4	5997	7	NULL	NULL	NULL	NULL	Ca2+	Chemical	low	induce					statement 3	Process	conformational changes of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
18833	5	5997	7	NULL	NULL	NULL	NULL	calpain	GP	active	undergoes					autoproteolysis	Process	irreversible			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
18834	6	5997	7	NULL	NULL	NULL	NULL	Ca2+	Chemical	high	produce					calpain	GP	soluble active native			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
18835	7	5997	7	NULL	NULL	NULL	NULL	calpain	GP	soluble active	associate with					plasma membrane	CellComponent	inner surface of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
18836	8	5997	7	NULL	NULL	NULL	NULL	calpain	GP	autoproteolyzed active	release from					plasma membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
18837	9	5997	7	NULL	NULL	NULL	NULL	Ca2+	Chemical	high	autoproteolyse					calpain	GP	active native			NULL	cytosol	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
18838	10	5997	7	NULL	NULL	NULL	NULL	calpastatin	GP		binds		high affinity			calpain	GP	active autoproteolyzed 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
18839	11	5997	7	NULL	NULL	NULL	NULL	calpastatin	GP		inhibits					calpain	GP	catalytic activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
18840	12	5997	7	NULL	NULL	NULL	NULL	calpastatin	GP		degrades					calpain	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
18841	13	5997	7	NULL	NULL	NULL	NULL	statement 12	Process		produce					active fragments	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
18842	14	5997	7	NULL	NULL	NULL	NULL	statement 12	Process		produce					inactive fragments	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
18843	15	5997	7	NULL	NULL	NULL	NULL	statement 13	Process		occurs along with					statement 14	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38426_s_200	11485997	, Ca2+-induced reversible association of inactive native calpain ( ellipsoid) to plasma membrane;  , low Ca2+-induced conformational changes producing active native calpain ( hexagon) onto the inner surface of the plasma membrane;  , irreversible autoproteolysis of active calpain ( pentagon);   , high Ca2+-induced conformational changes producing soluble active native calpain;   , possible association of soluble active calpain to the inner surface of plasma membrane;   , spontaneous release of autoproteolyzed active calpain ( pentagon) from the plasma membrane;   , possible (high Ca2+-requiring) autoproteolysis of active native calpain in cytosol;   , calpastatin ( cross) binds active autoproteolyzed calpain with high affinity, inhibiting its catalytic activity, and is also degraded, producing active and inactive fragments;   , calpastatin binds active native calpain, inhibiting its catalytic activity, and is degraded to active and inactive fragments at a lower rate.	bind
15681	1	5999	5	NULL	NULL	0	NULL	cytohesin-1	NULL		bind	NULL				GST-p3(24-30ARF1)	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_28_21331_s_188	10748148	, densitometry showed that binding of cytohesin-1 and cytohesin-2 to GST-p3(24-30ARF1) was only ~60% of that of cytohesin-1 to GST-p3.	bind
15682	2	5999	5	NULL	NULL	0	NULL	cytohesin-2	NULL		bind	NULL				GST-p3(24-30ARF1)	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_28_21331_s_188	10748148	, densitometry showed that binding of cytohesin-1 and cytohesin-2 to GST-p3(24-30ARF1) was only ~60% of that of cytohesin-1 to GST-p3.	bind
15683	3	5999	5	NULL	NULL	0	NULL	cytohesin-1	NULL		bind	NULL				GST-p3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_28_21331_s_188	10748148	, densitometry showed that binding of cytohesin-1 and cytohesin-2 to GST-p3(24-30ARF1) was only ~60% of that of cytohesin-1 to GST-p3.	bind
18513	1	5999	7	NULL	NULL	NULL	NULL	cytohesin-1	GP		bind					GST-p3 (24-30ARF1)	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_28_21331_s_188	10748148	, densitometry showed that binding of cytohesin-1 and cytohesin-2 to GST-p3(24-30ARF1) was only ~60% of that of cytohesin-1 to GST-p3.	bind
18515	2	5999	7	NULL	NULL	NULL	NULL	cytohesin-2	GP		bind					GST-p3(24-30ARF1) 	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_28_21331_s_188	10748148	, densitometry showed that binding of cytohesin-1 and cytohesin-2 to GST-p3(24-30ARF1) was only ~60% of that of cytohesin-1 to GST-p3.	bind
18518	3	5999	7	NULL	NULL	NULL	NULL	cytohesin-1	GP		bind					GST-p3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_28_21331_s_188	10748148	, densitometry showed that binding of cytohesin-1 and cytohesin-2 to GST-p3(24-30ARF1) was only ~60% of that of cytohesin-1 to GST-p3.	bind
15684	1	6001	5	NULL	NULL	0	NULL	GS I	NULL		interacts with	NULL				ovalbumin	NULL	pegion			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_17_14996_s_139	11836253	, laminin; +, bovine thyroglobulin;  ,  C. alata galactomannan;  , pigeon ovalbumin;  , GalNAcalpha1,3Galbeta polyacrylamide;  , GS I interaction with pigeon ovalbumin;  , GS I interaction with GalNAcalpha1,3Galbeta-polyacrylamide.	bind
15685	2	6001	5	NULL	NULL	0	NULL	GS I	NULL		interacts with	NULL				GalNAcalpha1,3Galbeta-polyacrylamide	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_17_14996_s_139	11836253	, laminin; +, bovine thyroglobulin;  ,  C. alata galactomannan;  , pigeon ovalbumin;  , GalNAcalpha1,3Galbeta polyacrylamide;  , GS I interaction with pigeon ovalbumin;  , GS I interaction with GalNAcalpha1,3Galbeta-polyacrylamide.	bind
18522	1	6001	7	NULL	NULL	NULL	NULL	GS I	GP		interacts with					ovalbumin	GP	pigeon			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_14996_s_139	11836253	, laminin; +, bovine thyroglobulin;  ,  C. alata galactomannan;  , pigeon ovalbumin;  , GalNAcalpha1,3Galbeta polyacrylamide;  , GS I interaction with pigeon ovalbumin;  , GS I interaction with GalNAcalpha1,3Galbeta-polyacrylamide.	bind
18523	2	6001	7	NULL	NULL	NULL	NULL	GS I	GP		interacts with					GalNAcalpha1,3Galbeta polyacrylamide	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_14996_s_139	11836253	, laminin; +, bovine thyroglobulin;  ,  C. alata galactomannan;  , pigeon ovalbumin;  , GalNAcalpha1,3Galbeta polyacrylamide;  , GS I interaction with pigeon ovalbumin;  , GS I interaction with GalNAcalpha1,3Galbeta-polyacrylamide.	bind
15686	1	6004	5	NULL	NULL	0	NULL	rGal-1 	NULL		bind	NULL				asialofetuin	NULL				NULL	in reducing buffer	0	NULL	NULL	NULL	gw60_jbiolchem_270_10_5198_s_149	7890630	, rGal-1 bound to asialofetuin-Sepharose in reducing buffer;   , rGal-1 bound to asialofetuin-Sepharose in nonreducing buffer;   , rGal-1 bound to laminin-Sepharose in nonreducing buffer;   , C2SrGal-1 bound to asialofetuin-Sepharose in nonreducing  buffer.	bind
15687	2	6004	5	NULL	NULL	0	NULL	rGal-1	NULL		bind	NULL				asialofetuin	NULL				NULL	in nonreducing buffer	0	NULL	NULL	NULL	gw60_jbiolchem_270_10_5198_s_149	7890630	, rGal-1 bound to asialofetuin-Sepharose in reducing buffer;   , rGal-1 bound to asialofetuin-Sepharose in nonreducing buffer;   , rGal-1 bound to laminin-Sepharose in nonreducing buffer;   , C2SrGal-1 bound to asialofetuin-Sepharose in nonreducing  buffer.	bind
15688	3	6004	5	NULL	NULL	0	NULL	rGal-1	NULL		bind	NULL				laminin	NULL				NULL	in reducing buffer	0	NULL	NULL	NULL	gw60_jbiolchem_270_10_5198_s_149	7890630	, rGal-1 bound to asialofetuin-Sepharose in reducing buffer;   , rGal-1 bound to asialofetuin-Sepharose in nonreducing buffer;   , rGal-1 bound to laminin-Sepharose in nonreducing buffer;   , C2SrGal-1 bound to asialofetuin-Sepharose in nonreducing  buffer.	bind
15689	4	6004	5	NULL	NULL	0	NULL	C2SrGal-1	NULL		bind	NULL				asialofetuin	NULL				NULL	in nonreducing buffer	0	NULL	NULL	NULL	gw60_jbiolchem_270_10_5198_s_149	7890630	, rGal-1 bound to asialofetuin-Sepharose in reducing buffer;   , rGal-1 bound to asialofetuin-Sepharose in nonreducing buffer;   , rGal-1 bound to laminin-Sepharose in nonreducing buffer;   , C2SrGal-1 bound to asialofetuin-Sepharose in nonreducing  buffer.	bind
18530	1	6004	7	NULL	NULL	NULL	NULL	 rGal-1	GP		bind					asialofetuin-Sepharose	Chemical				NULL	in reducing buffer	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_10_5198_s_149	7890630	, rGal-1 bound to asialofetuin-Sepharose in reducing buffer;   , rGal-1 bound to asialofetuin-Sepharose in nonreducing buffer;   , rGal-1 bound to laminin-Sepharose in nonreducing buffer;   , C2SrGal-1 bound to asialofetuin-Sepharose in nonreducing  buffer.	bind
18538	2	6004	7	NULL	NULL	NULL	NULL	rGal-1	GP		bind					asialofetuin-Sepharose	Chemical				NULL	in nonreducing buffer	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_10_5198_s_149	7890630	, rGal-1 bound to asialofetuin-Sepharose in reducing buffer;   , rGal-1 bound to asialofetuin-Sepharose in nonreducing buffer;   , rGal-1 bound to laminin-Sepharose in nonreducing buffer;   , C2SrGal-1 bound to asialofetuin-Sepharose in nonreducing  buffer.	bind
18539	3	6004	7	NULL	NULL	NULL	NULL	rGal-1	GP		bind					laminin-Sepharose	Chemical				NULL	in nonreducing buffer	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_10_5198_s_149	7890630	, rGal-1 bound to asialofetuin-Sepharose in reducing buffer;   , rGal-1 bound to asialofetuin-Sepharose in nonreducing buffer;   , rGal-1 bound to laminin-Sepharose in nonreducing buffer;   , C2SrGal-1 bound to asialofetuin-Sepharose in nonreducing  buffer.	bind
18540	4	6004	7	NULL	NULL	NULL	NULL	C2SrGal-1	GP		bind					asialofetuin-Sepharose	Chemical				NULL	in nonreducing buffer	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_10_5198_s_149	7890630	, rGal-1 bound to asialofetuin-Sepharose in reducing buffer;   , rGal-1 bound to asialofetuin-Sepharose in nonreducing buffer;   , rGal-1 bound to laminin-Sepharose in nonreducing buffer;   , C2SrGal-1 bound to asialofetuin-Sepharose in nonreducing  buffer.	bind
15690	1	6005	5	NULL	NULL	0	NULL	Quaternary ligand	NULL		bind	NULL				acetylcholinesterase	NULL		aromatic residues in active-site gorge		NULL		0	NULL	NULL	NULL	gw60_molpharmacol_55_6_982_s_293	10347238	, Schalk I, Ehret-Sabatier L, Bouet F, Goeldner M, Hirth C, Axelsen PH, Silman I and Sussman JL (1993) Quaternary ligand binding to aromatic residues in the active-site gorge of acetylcholinesterase.	bind
18542	1	6005	7	NULL	NULL	NULL	NULL	Quaternary ligand	Chemical		bind					acetylcholinesterase	GP		aromatic residues in the active-site gorge of 		NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_55_6_982_s_293	10347238	, Schalk I, Ehret-Sabatier L, Bouet F, Goeldner M, Hirth C, Axelsen PH, Silman I and Sussman JL (1993) Quaternary ligand binding to aromatic residues in the active-site gorge of acetylcholinesterase.	bind
15691	1	6009	5	NULL	NULL	0	NULL	GST-Six3	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_17_3_368_s_147	12569128	, the binding complex of GST-Six3 and DNA; arrowhead, supershifted binding complex using anti-Six3 antibody; arrow, supershifted binding complex using anti-GST antibody.	bind
18544	1	6009	7	NULL	NULL	NULL	NULL	GST-Six3	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_3_368_s_147	12569128	, the binding complex of GST-Six3 and DNA; arrowhead, supershifted binding complex using anti-Six3 antibody; arrow, supershifted binding complex using anti-GST antibody.	bind
15692	1	6010	5	NULL	NULL	0	NULL	oxipurinol	NULL		bind	NULL				xanthine oxidase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_14_7816_s_148	7713871	, without xanthine  oxidase (control);  , 2 muM  free xanthine oxidase;   , 2 muM  oxipurinol bound xanthine  oxidase.	bind
18545	1	6010	7	NULL	NULL	NULL	NULL	oxipurinol	Chemical		bind					xanthine oxidase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_14_7816_s_148	7713871	, without xanthine  oxidase (control);  , 2 muM  free xanthine oxidase;   , 2 muM  oxipurinol bound xanthine  oxidase.	bind
15693	1	6012	5	NULL	NULL	0	NULL	Abeta42	NULL		bind	NULL	state-specific 			Fe(II)	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_free-radic-biol-med_40_4_16458186_s_5	16458186	- and that Abeta42 influenced Fenton chemistry  through aggregation state-specific binding of both Fe(II) and Fe(III).	bind
15694	2	6012	5	NULL	NULL	0	NULL	Abeta42	NULL		bind	NULL	state-specific			Fe(III)	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_free-radic-biol-med_40_4_16458186_s_5	16458186	- and that Abeta42 influenced Fenton chemistry  through aggregation state-specific binding of both Fe(II) and Fe(III).	bind
15695	3	6012	5	NULL	NULL	0	NULL	Abeta42	NULL		influence	NULL				Fenton chemistry	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_free-radic-biol-med_40_4_16458186_s_5	16458186	- and that Abeta42 influenced Fenton chemistry  through aggregation state-specific binding of both Fe(II) and Fe(III).	bind
15696	4	6012	5	NULL	NULL	0	NULL	statement 3	NULL		occurs through	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_free-radic-biol-med_40_4_16458186_s_5	16458186	- and that Abeta42 influenced Fenton chemistry  through aggregation state-specific binding of both Fe(II) and Fe(III).	bind
15697	5	6012	5	NULL	NULL	0	NULL	statement 3	NULL		occurs through	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_free-radic-biol-med_40_4_16458186_s_5	16458186	- and that Abeta42 influenced Fenton chemistry  through aggregation state-specific binding of both Fe(II) and Fe(III).	bind
18546	1	6012	7	NULL	NULL	NULL	NULL	Abeta42	GP		bind		state-specific			Fe(II)	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_free-radic-biol-med_40_4_16458186_s_5	16458186	- and that Abeta42 influenced Fenton chemistry  through aggregation state-specific binding of both Fe(II) and Fe(III).	bind
18547	2	6012	7	NULL	NULL	NULL	NULL	Abeta42	GP		bind		state-specific			Fe(III)	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_free-radic-biol-med_40_4_16458186_s_5	16458186	- and that Abeta42 influenced Fenton chemistry  through aggregation state-specific binding of both Fe(II) and Fe(III).	bind
25484	3	6012	7	NULL	NULL	NULL	NULL	Abeta42	GP		influence					Fenton chemistry	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_free-radic-biol-med_40_4_16458186_s_5	16458186	- and that Abeta42 influenced Fenton chemistry  through aggregation state-specific binding of both Fe(II) and Fe(III).	bind
25485	4	6012	7	NULL	NULL	NULL	NULL	statement 3	Process		occurs through					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_free-radic-biol-med_40_4_16458186_s_5	16458186	- and that Abeta42 influenced Fenton chemistry  through aggregation state-specific binding of both Fe(II) and Fe(III).	bind
25486	5	6012	7	NULL	NULL	NULL	NULL	statement 3	Process		occurs through					statement 2	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_free-radic-biol-med_40_4_16458186_s_5	16458186	- and that Abeta42 influenced Fenton chemistry  through aggregation state-specific binding of both Fe(II) and Fe(III).	bind
15698	1	6013	5	NULL	NULL	0	NULL	PLN1-26-PDZ-Myc-His6	NULL		bind	NULL				GST-SERCA2LCL	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_3_667_s_144	11854448	-, Mg2+- and ATP-binding protein, we examined the effects of Ca2+, Mg2+ and ATP on the binding of PLN1-26-PDZ-Myc-His6 to GST-SERCA2LCL.	bind
18548	1	6013	7	NULL	NULL	NULL	NULL	PLN1-26-PDZ-Myc-His6 	GP		bind					GST-SERCA2LCL	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_61_3_667_s_144	11854448	-, Mg2+- and ATP-binding protein, we examined the effects of Ca2+, Mg2+ and ATP on the binding of PLN1-26-PDZ-Myc-His6 to GST-SERCA2LCL.	bind
15699	1	6014	5	NULL	NULL	0	NULL	fbf	NULL		bind	NULL	specifically			gld-3S	NULL			3''-UTR	NULL		0	NULL	NULL	NULL	gw70_genetics_168_1_147_s_289	15454534	--   fbf binds specifically to  gld-3S 3''-UTR.	bind
18549	1	6014	7	NULL	NULL	NULL	NULL	fbf	GP		bind		specifically			gld-3S 	GP			3''-UTR	NULL		NULL	NULL	NULL	NULL	gw70_genetics_168_1_147_s_289	15454534	--   fbf binds specifically to  gld-3S 3''-UTR.	bind
15700	1	6015	5	10	NULL	0	NULL	p47	NULL		bind	NULL				rbcL RNA	NULL	amaranth			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_5_3476_s_253	11076953	--  Although binding of p47 to amaranth  rbcL RNA was not competed with amaranth  psbA transcript, this binding activity does share some properties with light-associated proteins that interact with the 5''-UTR of  psbA mRNA in other plant systems ( 1-4).	bind
15701	2	6015	5	10	NULL	0	NULL	p47	NULL		bind	NULL				psbA transcript	NULL	amaranth			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_5_3476_s_253	11076953	--  Although binding of p47 to amaranth  rbcL RNA was not competed with amaranth  psbA transcript, this binding activity does share some properties with light-associated proteins that interact with the 5''-UTR of  psbA mRNA in other plant systems ( 1-4).	bind
15702	3	6015	5	10	NULL	0	NULL	light-associated proteins	NULL		interacts with	NULL				psbA mRNA	NULL			5''-UTR	NULL	in other plant systems	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_5_3476_s_253	11076953	--  Although binding of p47 to amaranth  rbcL RNA was not competed with amaranth  psbA transcript, this binding activity does share some properties with light-associated proteins that interact with the 5''-UTR of  psbA mRNA in other plant systems ( 1-4).	bind
54139	4	6015	5	10	NULL	0	NULL	statement 1			does not compete with					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_5_3476_s_253	11076953	--  Although binding of p47 to amaranth  rbcL RNA was not competed with amaranth  psbA transcript, this binding activity does share some properties with light-associated proteins that interact with the 5''-UTR of  psbA mRNA in other plant systems ( 1-4).	bind
18550	1	6015	7	NULL	NULL	NULL	NULL	p47	GP		bind					rbcL RNA	NucleicAcid	 amaranth			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_5_3476_s_253	11076953	--  Although binding of p47 to amaranth  rbcL RNA was not competed with amaranth  psbA transcript, this binding activity does share some properties with light-associated proteins that interact with the 5''-UTR of  psbA mRNA in other plant systems ( 1-4).	bind
18551	4	6015	7	NULL	NULL	NULL	NULL	statement 2	Process		does not compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_5_3476_s_253	11076953	--  Although binding of p47 to amaranth  rbcL RNA was not competed with amaranth  psbA transcript, this binding activity does share some properties with light-associated proteins that interact with the 5''-UTR of  psbA mRNA in other plant systems ( 1-4).	bind
18552	3	6015	7	NULL	NULL	NULL	NULL	light-associated proteins	GP		interact with					 psbA mRNA	NucleicAcid			5''-UTR	NULL	in other plant systems	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_5_3476_s_253	11076953	--  Although binding of p47 to amaranth  rbcL RNA was not competed with amaranth  psbA transcript, this binding activity does share some properties with light-associated proteins that interact with the 5''-UTR of  psbA mRNA in other plant systems ( 1-4).	bind
55018	2	6015	7	NULL	NULL	NULL	NULL	p47	GP		bind					psbA transcript	NucleicAcid	amaranth			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_5_3476_s_253	11076953	--  Although binding of p47 to amaranth  rbcL RNA was not competed with amaranth  psbA transcript, this binding activity does share some properties with light-associated proteins that interact with the 5''-UTR of  psbA mRNA in other plant systems ( 1-4).	bind
15703	1	6017	5	NULL	NULL	0	NULL	TBP	NULL		bind	NULL				INO1	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_genetics_169_4_1957_s_243	15716495	--  ChIP analysis of TBP binding to the  INO1 promoter.	bind
18553	1	6017	7	NULL	NULL	NULL	NULL	TBP	GP		bind					INO1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_genetics_169_4_1957_s_243	15716495	--  ChIP analysis of TBP binding to the  INO1 promoter.	bind
15704	1	6018	5	NULL	NULL	0	NULL	Fob1p	NULL		bind	NULL				RFB	NULL				NULL		NULL	NULL	NULL	NULL	gw70_genetics_168_3_1205_s_244	15579680	--  Fob1p binding to the RFB is not diminished in  rrm3delta134-196 cells.	bind
15705	2	6018	5	NULL	NULL	0	NULL	statement 1	NULL		is not diminished in	NULL				rrm3delta134-196 cells	NULL				NULL		0	NULL	NULL	NULL	gw70_genetics_168_3_1205_s_244	15579680	--  Fob1p binding to the RFB is not diminished in  rrm3delta134-196 cells.	bind
18554	1	6018	7	NULL	NULL	NULL	NULL	Fob1p	GP		bind					RFB	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_genetics_168_3_1205_s_244	15579680	--  Fob1p binding to the RFB is not diminished in  rrm3delta134-196 cells.	bind
18555	2	6018	7	NULL	NULL	NULL	NULL	statement 1	Process		is not diminished in					rrm3delta134-196 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_genetics_168_3_1205_s_244	15579680	--  Fob1p binding to the RFB is not diminished in  rrm3delta134-196 cells.	bind
15706	1	6019	5	NULL	NULL	0	NULL	GLD-3	NULL		bind	NULL		N terminus		GLD-2	NULL				NULL		0	NULL	NULL	NULL	gw70_genetics_168_1_147_s_173	15454534	--  GLD-3 N terminus binds to GLD-2.	bind
18556	1	6019	7	NULL	NULL	NULL	NULL	GLD-3	GP		binds			N terminus		GLD-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_genetics_168_1_147_s_173	15454534	--  GLD-3 N terminus binds to GLD-2.	bind
15707	1	6020	5	NULL	NULL	0	NULL	Hap1	NULL		bind	NULL				HAP1	NULL			promoter region - 50 to - 300	NULL		0	NULL	NULL	NULL	gw70_genetics_169_3_1343_s_81	15654089	--  Hap1 binding to the  HAP1 promoter region encompassing nucleotide sequence  - 50 to  - 300.	bind
18557	1	6020	7	NULL	NULL	NULL	NULL	Hap1	GP		bind					HAP1	GP			promoter region - 50 to - 300	NULL		NULL	NULL	NULL	NULL	gw70_genetics_169_3_1343_s_81	15654089	--  Hap1 binding to the  HAP1 promoter region encompassing nucleotide sequence  - 50 to  - 300.	bind
15708	1	6021	5	NULL	NULL	0	NULL	Rad53	NULL		bind	NULL		kinase domain		ARS1	NULL				NULL		0	NULL	NULL	NULL	gw70_genetics_174_1_87_s_198	16816422	--  Rad53 kinase domain binds ARS1.	bind
18558	1	6021	7	NULL	NULL	NULL	NULL	Rad53 	GP		binds			kinase domain		ARS1	GP				NULL		NULL	NULL	NULL	NULL	gw70_genetics_174_1_87_s_198	16816422	--  Rad53 kinase domain binds ARS1.	bind
15709	1	6022	5	10	NULL	0	NULL	Rgt1 	NULL		bind	NULL	constitutively			HXT1	NULL			promoter	NULL		NULL	NULL	NULL	NULL	gw70_genetics_169_2_583_s_103	15489524	--  Rgt1 constitutive repressors bind constitutively to the  HXT1 promoter.	bind
44814	2	6022	5	10	NULL	0	NULL	Rgt1	NULL		is a type of	NULL				constitutive repressor	NULL				NULL		NULL	NULL	NULL	NULL	gw70_genetics_169_2_583_s_103	15489524	--  Rgt1 constitutive repressors bind constitutively to the  HXT1 promoter.	bind
18559	1	6022	7	NULL	NULL	NULL	NULL	Rgt1	GP		bind		constitutively			HXT1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_genetics_169_2_583_s_103	15489524	--  Rgt1 constitutive repressors bind constitutively to the  HXT1 promoter.	bind
44817	2	6022	7	NULL	NULL	NULL	NULL	Rgt1	GP		is a type of					constitutive repressor	GP				NULL		NULL	NULL	NULL	NULL	gw70_genetics_169_2_583_s_103	15489524	--  Rgt1 constitutive repressors bind constitutively to the  HXT1 promoter.	bind
15710	1	6023	5	NULL	NULL	0	NULL	Rvs167p	NULL		bind	NULL		SH3 domain		Gyp5p	NULL				NULL		0	NULL	NULL	NULL	gw70_genetics_170_2_555_s_102	15802519	--  Rvs167p SH3 domain binds to Gyp5p and Gyl1p.	bind
15711	2	6023	5	NULL	NULL	0	NULL	Rvs167p	NULL		bind	NULL		SH3 domain		Gyl1p	NULL				NULL		0	NULL	NULL	NULL	gw70_genetics_170_2_555_s_102	15802519	--  Rvs167p SH3 domain binds to Gyp5p and Gyl1p.	bind
18560	1	6023	7	NULL	NULL	NULL	NULL	Rvs167p 	GP		bind			SH3 domain		Gyp5p	GP				NULL		NULL	NULL	NULL	NULL	gw70_genetics_170_2_555_s_102	15802519	--  Rvs167p SH3 domain binds to Gyp5p and Gyl1p.	bind
18561	2	6023	7	NULL	NULL	NULL	NULL	Rvs167p 	GP		bind			SH3 domain		Gyl1p	GP				NULL		NULL	NULL	NULL	NULL	gw70_genetics_170_2_555_s_102	15802519	--  Rvs167p SH3 domain binds to Gyp5p and Gyl1p.	bind
15712	1	6024	5	10	NULL	0	NULL	SEM-5/Grb2	NULL		bind	NULL		C-terminal SH3 domain		SOC-1/Gab1	NULL	atypical	proline-rich motif		NULL		NULL	NULL	NULL	NULL	gw70_genetics_173_1_163_s_116	16547100	--  The C-terminal SH3 domain of SEM-5/Grb2 binds an atypical proline-rich motif  within SOC-1/Gab1.	bind
18562	1	6024	7	NULL	NULL	NULL	NULL	SEM-5/Grb2	GP		binds to			C-terminal SH3 domain 		SOC-1/Gab1	GP		proline-rich motif		NULL		NULL	NULL	NULL	NULL	gw70_genetics_173_1_163_s_116	16547100	--  The C-terminal SH3 domain of SEM-5/Grb2 binds an atypical proline-rich motif  within SOC-1/Gab1.	bind
15714	1	6026	5	10	NULL	0	NULL	E1A	NULL		bind	NULL				CtBP 	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_41_38755_s_277	12161448	-- A previous report indicated that acetylation of E1A might diminish binding to the CtBP co-repressor ( 34) in contrast to this study.	bind
25642	2	6026	5	NULL	NULL	0	NULL	E1A	NULL	acetylation of	diminish	NULL	might			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_41_38755_s_277	12161448	-- A previous report indicated that acetylation of E1A might diminish binding to the CtBP co-repressor ( 34) in contrast to this study.	bind
44818	3	6026	5	10	NULL	0	NULL	CtBP	NULL		is a type of	NULL				co-repressor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_41_38755_s_277	12161448	-- A previous report indicated that acetylation of E1A might diminish binding to the CtBP co-repressor ( 34) in contrast to this study.	bind
18563	1	6026	7	NULL	NULL	NULL	NULL	E1A	GP		bind					CtBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_41_38755_s_277	12161448	-- A previous report indicated that acetylation of E1A might diminish binding to the CtBP co-repressor ( 34) in contrast to this study.	bind
18564	2	6026	7	NULL	NULL	NULL	NULL	E1A	GP	acetylation of	diminish		might			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_41_38755_s_277	12161448	-- A previous report indicated that acetylation of E1A might diminish binding to the CtBP co-repressor ( 34) in contrast to this study.	bind
44819	3	6026	7	NULL	NULL	NULL	NULL	CtBP	GP		is a type of					co-repressor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_41_38755_s_277	12161448	-- A previous report indicated that acetylation of E1A might diminish binding to the CtBP co-repressor ( 34) in contrast to this study.	bind
15715	1	6027	5	NULL	NULL	0	NULL	stigmatellin	NULL		bind	NULL				bc1 complex	NULL	native			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_5_3464_s_81	11707448	-- Binding of class II inhibitors like stigmatellin to the native  bc1 complex is known to increase the  Em value of the [2Fe-2S] cluster of the iron-sulfur subunit by about 200 mV ( 30).	bind
25643	2	6027	5	NULL	NULL	0	NULL	stigmatellin	NULL		is a type of	NULL				class II inhibitor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_5_3464_s_81	11707448	-- Binding of class II inhibitors like stigmatellin to the native  bc1 complex is known to increase the  Em value of the [2Fe-2S] cluster of the iron-sulfur subunit by about 200 mV ( 30).	bind
18565	1	6027	7	NULL	NULL	NULL	NULL	stigmatellin 	Chemical		bind					 bc1 complex	GP	native			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_5_3464_s_81	11707448	-- Binding of class II inhibitors like stigmatellin to the native  bc1 complex is known to increase the  Em value of the [2Fe-2S] cluster of the iron-sulfur subunit by about 200 mV ( 30).	bind
18567	2	6027	7	NULL	NULL	NULL	NULL	stigmatellin 	Chemical		is a type of					class II inhibitors	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_5_3464_s_81	11707448	-- Binding of class II inhibitors like stigmatellin to the native  bc1 complex is known to increase the  Em value of the [2Fe-2S] cluster of the iron-sulfur subunit by about 200 mV ( 30).	bind
15716	1	6028	5	NULL	NULL	0	NULL	Na+	NULL		bind	NULL				E1 form	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_50_50283_s_240	14522987	-- It is generally accepted that the high and low affinity ATP binding reflects, respectively, binding to the E1 and E2 conformational state and that Na+ binds to the E1 form preceding phosphorylation and K+ binds to the E2 form during the Na/K-ATPase and  pNPPase reaction ( ,  ).	bind
15717	2	6028	5	NULL	NULL	0	NULL	statement 1	NULL		precede	NULL				phosphorylation	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_50_50283_s_240	14522987	-- It is generally accepted that the high and low affinity ATP binding reflects, respectively, binding to the E1 and E2 conformational state and that Na+ binds to the E1 form preceding phosphorylation and K+ binds to the E2 form during the Na/K-ATPase and  pNPPase reaction ( ,  ).	bind
15718	3	6028	5	NULL	NULL	0	NULL	K+	NULL		bind	NULL				E2 form	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_50_50283_s_240	14522987	-- It is generally accepted that the high and low affinity ATP binding reflects, respectively, binding to the E1 and E2 conformational state and that Na+ binds to the E1 form preceding phosphorylation and K+ binds to the E2 form during the Na/K-ATPase and  pNPPase reaction ( ,  ).	bind
15719	4	6028	5	NULL	NULL	0	NULL	statement 3	NULL		occurs during	NULL				Na/K-ATPase	NULL	reaction of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_50_50283_s_240	14522987	-- It is generally accepted that the high and low affinity ATP binding reflects, respectively, binding to the E1 and E2 conformational state and that Na+ binds to the E1 form preceding phosphorylation and K+ binds to the E2 form during the Na/K-ATPase and  pNPPase reaction ( ,  ).	bind
15720	5	6028	5	NULL	NULL	0	NULL	statement 3	NULL		occurs during	NULL				pNPPase	NULL	reaction of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_50_50283_s_240	14522987	-- It is generally accepted that the high and low affinity ATP binding reflects, respectively, binding to the E1 and E2 conformational state and that Na+ binds to the E1 form preceding phosphorylation and K+ binds to the E2 form during the Na/K-ATPase and  pNPPase reaction ( ,  ).	bind
25645	6	6028	5	NULL	NULL	0	NULL	ATP	NULL		bind	NULL	high affinity			E1 conformational state	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_50_50283_s_240	14522987	-- It is generally accepted that the high and low affinity ATP binding reflects, respectively, binding to the E1 and E2 conformational state and that Na+ binds to the E1 form preceding phosphorylation and K+ binds to the E2 form during the Na/K-ATPase and  pNPPase reaction ( ,  ).	bind
25646	7	6028	5	NULL	NULL	0	NULL	ATP	NULL		bind	NULL	low affinity			E2 conformational state	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_50_50283_s_240	14522987	-- It is generally accepted that the high and low affinity ATP binding reflects, respectively, binding to the E1 and E2 conformational state and that Na+ binds to the E1 form preceding phosphorylation and K+ binds to the E2 form during the Na/K-ATPase and  pNPPase reaction ( ,  ).	bind
18568	1	6028	7	NULL	NULL	NULL	NULL	ATP	Chemical		bind		high affinity			E1 conformational state	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_50_50283_s_240	14522987	-- It is generally accepted that the high and low affinity ATP binding reflects, respectively, binding to the E1 and E2 conformational state and that Na+ binds to the E1 form preceding phosphorylation and K+ binds to the E2 form during the Na/K-ATPase and  pNPPase reaction ( ,  ).	bind
18569	2	6028	7	NULL	NULL	NULL	NULL	ATP	Chemical		bind		low affinity			E2 conformational state	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_50_50283_s_240	14522987	-- It is generally accepted that the high and low affinity ATP binding reflects, respectively, binding to the E1 and E2 conformational state and that Na+ binds to the E1 form preceding phosphorylation and K+ binds to the E2 form during the Na/K-ATPase and  pNPPase reaction ( ,  ).	bind
18570	3	6028	7	NULL	NULL	NULL	NULL	Na+	Chemical		binds to					E1 form	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_50_50283_s_240	14522987	-- It is generally accepted that the high and low affinity ATP binding reflects, respectively, binding to the E1 and E2 conformational state and that Na+ binds to the E1 form preceding phosphorylation and K+ binds to the E2 form during the Na/K-ATPase and  pNPPase reaction ( ,  ).	bind
18571	4	6028	7	NULL	NULL	NULL	NULL	K+	Chemical		binds to					E2 form	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_50_50283_s_240	14522987	-- It is generally accepted that the high and low affinity ATP binding reflects, respectively, binding to the E1 and E2 conformational state and that Na+ binds to the E1 form preceding phosphorylation and K+ binds to the E2 form during the Na/K-ATPase and  pNPPase reaction ( ,  ).	bind
18572	5	6028	7	NULL	NULL	NULL	NULL	statement 3	Process		occurs preceding					phosphorylation	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_50_50283_s_240	14522987	-- It is generally accepted that the high and low affinity ATP binding reflects, respectively, binding to the E1 and E2 conformational state and that Na+ binds to the E1 form preceding phosphorylation and K+ binds to the E2 form during the Na/K-ATPase and  pNPPase reaction ( ,  ).	bind
18573	6	6028	7	NULL	NULL	NULL	NULL	statement 4	Process		occurs during					Na/K-ATPase	GP	reaction of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_50_50283_s_240	14522987	-- It is generally accepted that the high and low affinity ATP binding reflects, respectively, binding to the E1 and E2 conformational state and that Na+ binds to the E1 form preceding phosphorylation and K+ binds to the E2 form during the Na/K-ATPase and  pNPPase reaction ( ,  ).	bind
18574	7	6028	7	NULL	NULL	NULL	NULL	statement 4	Process		occurs during					pNPPase	GP	reaction of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_50_50283_s_240	14522987	-- It is generally accepted that the high and low affinity ATP binding reflects, respectively, binding to the E1 and E2 conformational state and that Na+ binds to the E1 form preceding phosphorylation and K+ binds to the E2 form during the Na/K-ATPase and  pNPPase reaction ( ,  ).	bind
15721	1	6029	5	NULL	NULL	0	NULL	p21	NULL		does not bind	NULL				PCNA	NULL				NULL	during arrest	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_5802_s_249	14597617	-- One striking observation was the fact that p21 does not bind to PCNA during arrest.	bind
18575	1	6029	7	NULL	NULL	NULL	NULL	 p21	GP		does not bind					PCNA	GP				NULL	during arrest	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_5802_s_249	14597617	-- One striking observation was the fact that p21 does not bind to PCNA during arrest.	bind
15722	1	6030	5	NULL	NULL	0	NULL	heparin	NULL		bind	NULL				vitronectin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_10_6432_s_338	10037735	-- Previous work from this laboratory had demonstrated that the dissociation constant for the binding of heparin to vitronectin was dependent on ionic strength ( 23).	bind
18576	1	6030	7	NULL	NULL	NULL	NULL	heparin	GP		bind					vitronectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_10_6432_s_338	10037735	-- Previous work from this laboratory had demonstrated that the dissociation constant for the binding of heparin to vitronectin was dependent on ionic strength ( 23).	bind
19062	1	6032	5	NULL	NULL	0	NULL		NULL		lies on	NULL		GABA binding site			NULL		interface of the alpha and beta subunits		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_38_26633_s_179	10480864	-- Since the GABA binding site lies on the interface of the alpha and beta subunits, and since the mutant alpha1 subunits expressed with the beta2 subunits bind [3]muscimol, the GABA binding interface is unaffected by the Trp-69 and Trp-94 mutations.	bind
19078	2	6032	5	NULL	NULL	0	NULL		NULL	mutant	is expressed with	NULL		alpha1 subunits			NULL		beta2 subunits		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_38_26633_s_179	10480864	-- Since the GABA binding site lies on the interface of the alpha and beta subunits, and since the mutant alpha1 subunits expressed with the beta2 subunits bind [3]muscimol, the GABA binding interface is unaffected by the Trp-69 and Trp-94 mutations.	bind
19079	4	6032	5	NULL	NULL	0	NULL		NULL		is unaffected by	NULL		GABA binding interface			NULL	mutation of	Trp-69		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_38_26633_s_179	10480864	-- Since the GABA binding site lies on the interface of the alpha and beta subunits, and since the mutant alpha1 subunits expressed with the beta2 subunits bind [3]muscimol, the GABA binding interface is unaffected by the Trp-69 and Trp-94 mutations.	bind
19080	5	6032	5	NULL	NULL	0	NULL		NULL		is unaffected by	NULL		GABA binding interface			NULL	mutation of	Trp-94		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_38_26633_s_179	10480864	-- Since the GABA binding site lies on the interface of the alpha and beta subunits, and since the mutant alpha1 subunits expressed with the beta2 subunits bind [3]muscimol, the GABA binding interface is unaffected by the Trp-69 and Trp-94 mutations.	bind
19191	3	6032	5	NULL	NULL	0	NULL	statement 2	NULL		bind	NULL				muscimol	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_38_26633_s_179	10480864	-- Since the GABA binding site lies on the interface of the alpha and beta subunits, and since the mutant alpha1 subunits expressed with the beta2 subunits bind [3]muscimol, the GABA binding interface is unaffected by the Trp-69 and Trp-94 mutations.	bind
18580	1	6032	7	NULL	NULL	0	NULL		NULL	mutant	expressed with	NULL		alpha1 subunit			NULL		beta2 subunits 		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_38_26633_s_179	10480864	-- Since the GABA binding site lies on the interface of the alpha and beta subunits, and since the mutant alpha1 subunits expressed with the beta2 subunits bind [3]muscimol, the GABA binding interface is unaffected by the Trp-69 and Trp-94 mutations.	bind
18581	2	6032	7	NULL	NULL	NULL	NULL	statement 1	Process		bind					muscimol	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_38_26633_s_179	10480864	-- Since the GABA binding site lies on the interface of the alpha and beta subunits, and since the mutant alpha1 subunits expressed with the beta2 subunits bind [3]muscimol, the GABA binding interface is unaffected by the Trp-69 and Trp-94 mutations.	bind
18582	3	6032	7	NULL	NULL	0	NULL		NULL		lies on	NULL		GABA binding site			NULL		the interface of alpha and beta subunits		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_38_26633_s_179	10480864	-- Since the GABA binding site lies on the interface of the alpha and beta subunits, and since the mutant alpha1 subunits expressed with the beta2 subunits bind [3]muscimol, the GABA binding interface is unaffected by the Trp-69 and Trp-94 mutations.	bind
18583	4	6032	7	NULL	NULL	0	NULL	 	NULL		is unaffected by	NULL		GABA binding interface			NULL	mutation of	Trp-69		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_38_26633_s_179	10480864	-- Since the GABA binding site lies on the interface of the alpha and beta subunits, and since the mutant alpha1 subunits expressed with the beta2 subunits bind [3]muscimol, the GABA binding interface is unaffected by the Trp-69 and Trp-94 mutations.	bind
18584	5	6032	7	NULL	NULL	0	NULL		NULL		is unaffected by	NULL		GABA binding interface			NULL	mutation of	Trp-94		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_38_26633_s_179	10480864	-- Since the GABA binding site lies on the interface of the alpha and beta subunits, and since the mutant alpha1 subunits expressed with the beta2 subunits bind [3]muscimol, the GABA binding interface is unaffected by the Trp-69 and Trp-94 mutations.	bind
15724	1	6033	5	NULL	NULL	0	NULL	HHR23A	NULL		bind	NULL		UBA domains		Ub	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11926_s_262	14707125	-- The chemical shift mapping study presented here reveals a structural basis for the recognition and binding of UBA domains of HHR23A to Ub.	bind
18585	1	6033	7	NULL	NULL	NULL	NULL	HHR23A	GP		binds to			UBA domain		Ub	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_12_11926_s_262	14707125	-- The chemical shift mapping study presented here reveals a structural basis for the recognition and binding of UBA domains of HHR23A to Ub.	bind
15725	1	6034	5	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				Cdc42	NULL	activated			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49293_s_135	14506284	-- We had previously shown that treatment of NIH 3T3 cells with EGF led to a relatively rapid increase in the levels of GTP-bound (activated) Cdc42 ( ), as read-out by an assay that examines the binding of this GTP-binding protein to its limit-binding domain on PAK (called the PBD).	bind
15726	2	6034	5	NULL	NULL	0	NULL	GTP-binding protein	NULL		bind	NULL				PAK	NULL		PBD		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49293_s_135	14506284	-- We had previously shown that treatment of NIH 3T3 cells with EGF led to a relatively rapid increase in the levels of GTP-bound (activated) Cdc42 ( ), as read-out by an assay that examines the binding of this GTP-binding protein to its limit-binding domain on PAK (called the PBD).	bind
25647	3	6034	5	NULL	NULL	0	NULL	NIH 3T3 cells	NULL		treated with	NULL				EGF	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49293_s_135	14506284	-- We had previously shown that treatment of NIH 3T3 cells with EGF led to a relatively rapid increase in the levels of GTP-bound (activated) Cdc42 ( ), as read-out by an assay that examines the binding of this GTP-binding protein to its limit-binding domain on PAK (called the PBD).	bind
25648	4	6034	5	NULL	NULL	0	NULL	statement 3	NULL		increases	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49293_s_135	14506284	-- We had previously shown that treatment of NIH 3T3 cells with EGF led to a relatively rapid increase in the levels of GTP-bound (activated) Cdc42 ( ), as read-out by an assay that examines the binding of this GTP-binding protein to its limit-binding domain on PAK (called the PBD).	bind
18586	1	6034	7	NULL	NULL	NULL	NULL	GTP	Chemical		bind					Cdc42	GP	activated			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49293_s_135	14506284	-- We had previously shown that treatment of NIH 3T3 cells with EGF led to a relatively rapid increase in the levels of GTP-bound (activated) Cdc42 ( ), as read-out by an assay that examines the binding of this GTP-binding protein to its limit-binding domain on PAK (called the PBD).	bind
18587	2	6034	7	NULL	NULL	NULL	NULL	GTP-binding protein	GP		bind					 PAK	GP		PBD		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49293_s_135	14506284	-- We had previously shown that treatment of NIH 3T3 cells with EGF led to a relatively rapid increase in the levels of GTP-bound (activated) Cdc42 ( ), as read-out by an assay that examines the binding of this GTP-binding protein to its limit-binding domain on PAK (called the PBD).	bind
18588	3	6034	7	NULL	NULL	NULL	NULL	NIH 3T3 cells	Cell		treated with					EGF	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49293_s_135	14506284	-- We had previously shown that treatment of NIH 3T3 cells with EGF led to a relatively rapid increase in the levels of GTP-bound (activated) Cdc42 ( ), as read-out by an assay that examines the binding of this GTP-binding protein to its limit-binding domain on PAK (called the PBD).	bind
25640	4	6034	7	NULL	NULL	NULL	NULL	statement 3	Process		increase					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49293_s_135	14506284	-- We had previously shown that treatment of NIH 3T3 cells with EGF led to a relatively rapid increase in the levels of GTP-bound (activated) Cdc42 ( ), as read-out by an assay that examines the binding of this GTP-binding protein to its limit-binding domain on PAK (called the PBD).	bind
15727	1	6037	5	NULL	NULL	0	NULL	Actinin	NULL		bind	NULL				Tir	NULL		amino terminus		NULL		0	NULL	NULL	NULL	gw60_currbiol_10_12_735_s_76	10873808	-Actinin binds the amino terminus of Tir	bind
18589	1	6037	7	NULL	NULL	NULL	NULL	Actinin	GP		binds					Tir	GP		amino terminus		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_12_735_s_76	10873808	-Actinin binds the amino terminus of Tir	bind
15728	1	6038	5	NULL	NULL	0	NULL	Actinin	NULL		is composed of	NULL					NULL		amino-terminal actin-binding region		NULL		0	NULL	NULL	NULL	gw60_cell_98_4_537_s_30	10481917	-Actinin is composed of an amino-terminal actin-binding  region consisting of two calponin homology (CH) domains, a central rod containing four spectrin-like  repeats, and a calmodulin-like domain at the carboxy terminus (Castresana and Saraste, 1995   ;  Trave et al., 1995   ;  Davison and Critchley, 1988   ).	bind
15729	2	6038	5	NULL	NULL	0	NULL		NULL		consists of	NULL		amino-terminal actin-binding region			NULL		two CH domains		NULL		NULL	NULL	NULL	NULL	gw60_cell_98_4_537_s_30	10481917	-Actinin is composed of an amino-terminal actin-binding  region consisting of two calponin homology (CH) domains, a central rod containing four spectrin-like  repeats, and a calmodulin-like domain at the carboxy terminus (Castresana and Saraste, 1995   ;  Trave et al., 1995   ;  Davison and Critchley, 1988   ).	bind
15730	3	6038	5	NULL	NULL	0	NULL	CH domain	NULL		is	NULL				calponin homology domain	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_98_4_537_s_30	10481917	-Actinin is composed of an amino-terminal actin-binding  region consisting of two calponin homology (CH) domains, a central rod containing four spectrin-like  repeats, and a calmodulin-like domain at the carboxy terminus (Castresana and Saraste, 1995   ;  Trave et al., 1995   ;  Davison and Critchley, 1988   ).	bind
15731	4	6038	5	NULL	NULL	0	NULL		NULL		consists of	NULL		amino-terminal actin-binding region			NULL	central rod containing	four spectrin-like repeats		NULL		0	NULL	NULL	NULL	gw60_cell_98_4_537_s_30	10481917	-Actinin is composed of an amino-terminal actin-binding  region consisting of two calponin homology (CH) domains, a central rod containing four spectrin-like  repeats, and a calmodulin-like domain at the carboxy terminus (Castresana and Saraste, 1995   ;  Trave et al., 1995   ;  Davison and Critchley, 1988   ).	bind
15732	5	6038	5	NULL	NULL	0	NULL		NULL		consists of	NULL		amino-terminal actin-binding region			NULL	at carboxy terminus	calmodulin-like domain		NULL		0	NULL	NULL	NULL	gw60_cell_98_4_537_s_30	10481917	-Actinin is composed of an amino-terminal actin-binding  region consisting of two calponin homology (CH) domains, a central rod containing four spectrin-like  repeats, and a calmodulin-like domain at the carboxy terminus (Castresana and Saraste, 1995   ;  Trave et al., 1995   ;  Davison and Critchley, 1988   ).	bind
18590	1	6038	7	NULL	NULL	NULL	NULL	Actinin	GP		is composed of								amino-terminal actin-binding region		NULL		NULL	NULL	NULL	NULL	gw60_cell_98_4_537_s_30	10481917	-Actinin is composed of an amino-terminal actin-binding  region consisting of two calponin homology (CH) domains, a central rod containing four spectrin-like  repeats, and a calmodulin-like domain at the carboxy terminus (Castresana and Saraste, 1995   ;  Trave et al., 1995   ;  Davison and Critchley, 1988   ).	bind
18591	2	6038	7	NULL	NULL	NULL	NULL	statement 1	Process		consist of								two CH domains		NULL		NULL	NULL	NULL	NULL	gw60_cell_98_4_537_s_30	10481917	-Actinin is composed of an amino-terminal actin-binding  region consisting of two calponin homology (CH) domains, a central rod containing four spectrin-like  repeats, and a calmodulin-like domain at the carboxy terminus (Castresana and Saraste, 1995   ;  Trave et al., 1995   ;  Davison and Critchley, 1988   ).	bind
18592	3	6038	7	NULL	NULL	NULL	NULL	Actinin	GP		is composed of							central rod containing	four spectrin-like repeats		NULL		NULL	NULL	NULL	NULL	gw60_cell_98_4_537_s_30	10481917	-Actinin is composed of an amino-terminal actin-binding  region consisting of two calponin homology (CH) domains, a central rod containing four spectrin-like  repeats, and a calmodulin-like domain at the carboxy terminus (Castresana and Saraste, 1995   ;  Trave et al., 1995   ;  Davison and Critchley, 1988   ).	bind
18593	4	6038	7	NULL	NULL	NULL	NULL	Actinin 	GP		is composed of								calmodulin-like domain at the carboxy terminus		NULL		NULL	NULL	NULL	NULL	gw60_cell_98_4_537_s_30	10481917	-Actinin is composed of an amino-terminal actin-binding  region consisting of two calponin homology (CH) domains, a central rod containing four spectrin-like  repeats, and a calmodulin-like domain at the carboxy terminus (Castresana and Saraste, 1995   ;  Trave et al., 1995   ;  Davison and Critchley, 1988   ).	bind
18594	5	6038	7	NULL	NULL	NULL	NULL	CH domain	GP		is					calponin homology domain					NULL		NULL	NULL	NULL	NULL	gw60_cell_98_4_537_s_30	10481917	-Actinin is composed of an amino-terminal actin-binding  region consisting of two calponin homology (CH) domains, a central rod containing four spectrin-like  repeats, and a calmodulin-like domain at the carboxy terminus (Castresana and Saraste, 1995   ;  Trave et al., 1995   ;  Davison and Critchley, 1988   ).	bind
15733	1	6039	5	NULL	NULL	0	NULL	arrestin2	NULL		bind	NULL				clathrin	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevcelldevbiol_15_0_705_s_275	10611976	-arrestin2 lacks this serine, however, and it is not clear  whether its binding to clathrin is similarly controlled.	bind
18595	1	6039	7	NULL	NULL	NULL	NULL	arrestin2	GP		bind					clathrin	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_15_0_705_s_275	10611976	-arrestin2 lacks this serine, however, and it is not clear  whether its binding to clathrin is similarly controlled.	bind
15734	1	6040	5	NULL	NULL	0	NULL	ATP	NULL		bind	NULL				PDI (3K)	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1479_1_293_s_195	11004547	-ATP bound to PDI      (3K)	bind
18596	1	6040	7	NULL	NULL	NULL	NULL	ATP	Chemical		bind					PDI	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1479_1_293_s_195	11004547	-ATP bound to PDI      (3K)	bind
15735	1	6041	5	NULL	NULL	0	NULL	ATP	NULL		bind	NULL				PDI	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1479_1_293_s_125	11004547	-ATP bound to PDI is responsible for the decrease in the efficiency of energy transfer reflected in the measured phosphorescence yield.	bind
18597	1	6041	7	NULL	NULL	NULL	NULL	ATP	Chemical		bind					PDI	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1479_1_293_s_125	11004547	-ATP bound to PDI is responsible for the decrease in the efficiency of energy transfer reflected in the measured phosphorescence yield.	bind
15736	1	6042	5	NULL	NULL	0	NULL	ATP	NULL		bind	NULL				PDI	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1479_1_293_s_112	11004547	-ATP bound to PDI, coordination of Tb3+ by carboxyl groups of the protein might influence the stability and phosphorescence properties of the bound ligand.	bind
25649	2	6042	5	10	NULL	0	NULL	Tb3+	NULL		coordinate	NULL		carboxyl groups		Tb3+	NULL				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1479_1_293_s_112	11004547	-ATP bound to PDI, coordination of Tb3+ by carboxyl groups of the protein might influence the stability and phosphorescence properties of the bound ligand.	bind
25650	3	6042	5	NULL	NULL	0	NULL	statement 2	NULL		influence	NULL				ligand	NULL	stability of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1479_1_293_s_112	11004547	-ATP bound to PDI, coordination of Tb3+ by carboxyl groups of the protein might influence the stability and phosphorescence properties of the bound ligand.	bind
25651	4	6042	5	NULL	NULL	0	NULL	statement 2	NULL		influence	NULL				ligand	NULL	phosphorescence properties of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1479_1_293_s_112	11004547	-ATP bound to PDI, coordination of Tb3+ by carboxyl groups of the protein might influence the stability and phosphorescence properties of the bound ligand.	bind
18682	1	6042	7	NULL	NULL	NULL	NULL	ATP	Chemical		bind					PDI	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1479_1_293_s_112	11004547	-ATP bound to PDI, coordination of Tb3+ by carboxyl groups of the protein might influence the stability and phosphorescence properties of the bound ligand.	bind
18685	2	6042	7	NULL	NULL	NULL	NULL	Tb3+	Chemical		coordinate			carboxyl groups		Tb3+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1479_1_293_s_112	11004547	-ATP bound to PDI, coordination of Tb3+ by carboxyl groups of the protein might influence the stability and phosphorescence properties of the bound ligand.	bind
18690	4	6042	7	NULL	NULL	NULL	NULL	statement 2	Process		influence					ligand	Chemical	phosphorescence properties of 			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1479_1_293_s_112	11004547	-ATP bound to PDI, coordination of Tb3+ by carboxyl groups of the protein might influence the stability and phosphorescence properties of the bound ligand.	bind
25641	3	6042	7	NULL	NULL	NULL	NULL	statement 2	Process		influence					ligand	Chemical	stability of			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1479_1_293_s_112	11004547	-ATP bound to PDI, coordination of Tb3+ by carboxyl groups of the protein might influence the stability and phosphorescence properties of the bound ligand.	bind
15737	1	6044	5	NULL	NULL	0	NULL	catenin	NULL		bind	NULL				S-SCAM	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_27_4_509_s_164	15555928	-catenin also binds to the scaffolding protein S-SCAM (MAGI-2) (  Nishimura et al., 2002) which binds a variety of postsynaptic molecules including neuroligin, GKAP/SAPAP,  and NMDA receptors as well as presynaptically localized m-Lin 7 (MALS, Velis) (  Perego et al., 2000).	bind
15738	2	6044	5	NULL	NULL	0	NULL	S-SCAM	NULL		is	NULL				MAGI-2	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellneurosci_27_4_509_s_164	15555928	-catenin also binds to the scaffolding protein S-SCAM (MAGI-2) (  Nishimura et al., 2002) which binds a variety of postsynaptic molecules including neuroligin, GKAP/SAPAP,  and NMDA receptors as well as presynaptically localized m-Lin 7 (MALS, Velis) (  Perego et al., 2000).	bind
15739	3	6044	5	NULL	NULL	0	NULL	S-SCAM	NULL		bind	NULL				neuroligin	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellneurosci_27_4_509_s_164	15555928	-catenin also binds to the scaffolding protein S-SCAM (MAGI-2) (  Nishimura et al., 2002) which binds a variety of postsynaptic molecules including neuroligin, GKAP/SAPAP,  and NMDA receptors as well as presynaptically localized m-Lin 7 (MALS, Velis) (  Perego et al., 2000).	bind
15740	4	6044	5	NULL	NULL	0	NULL	S-SCAM	NULL		bind	NULL				GKAP/SAPAP	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellneurosci_27_4_509_s_164	15555928	-catenin also binds to the scaffolding protein S-SCAM (MAGI-2) (  Nishimura et al., 2002) which binds a variety of postsynaptic molecules including neuroligin, GKAP/SAPAP,  and NMDA receptors as well as presynaptically localized m-Lin 7 (MALS, Velis) (  Perego et al., 2000).	bind
15741	5	6044	5	NULL	NULL	0	NULL	S-SCAM	NULL		bind	NULL				NMDA receptors	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellneurosci_27_4_509_s_164	15555928	-catenin also binds to the scaffolding protein S-SCAM (MAGI-2) (  Nishimura et al., 2002) which binds a variety of postsynaptic molecules including neuroligin, GKAP/SAPAP,  and NMDA receptors as well as presynaptically localized m-Lin 7 (MALS, Velis) (  Perego et al., 2000).	bind
15742	6	6044	5	NULL	NULL	0	NULL	S-SCAM	NULL		bind	NULL				m-Lin 7	NULL	presynaptically localized			NULL		0	NULL	NULL	NULL	gw70_molcellneurosci_27_4_509_s_164	15555928	-catenin also binds to the scaffolding protein S-SCAM (MAGI-2) (  Nishimura et al., 2002) which binds a variety of postsynaptic molecules including neuroligin, GKAP/SAPAP,  and NMDA receptors as well as presynaptically localized m-Lin 7 (MALS, Velis) (  Perego et al., 2000).	bind
25652	7	6044	5	NULL	NULL	0	NULL	S-SCAM	NULL		is a type of	NULL				scaffolding protein	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellneurosci_27_4_509_s_164	15555928	-catenin also binds to the scaffolding protein S-SCAM (MAGI-2) (  Nishimura et al., 2002) which binds a variety of postsynaptic molecules including neuroligin, GKAP/SAPAP,  and NMDA receptors as well as presynaptically localized m-Lin 7 (MALS, Velis) (  Perego et al., 2000).	bind
25653	8	6044	5	NULL	NULL	0	NULL	neuroligin	NULL		is a type of	NULL				postsynaptic molecule	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellneurosci_27_4_509_s_164	15555928	-catenin also binds to the scaffolding protein S-SCAM (MAGI-2) (  Nishimura et al., 2002) which binds a variety of postsynaptic molecules including neuroligin, GKAP/SAPAP,  and NMDA receptors as well as presynaptically localized m-Lin 7 (MALS, Velis) (  Perego et al., 2000).	bind
25654	9	6044	5	NULL	NULL	0	NULL	GKAP/SAPAP	NULL		is a type of	NULL				postsynaptic molecule	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellneurosci_27_4_509_s_164	15555928	-catenin also binds to the scaffolding protein S-SCAM (MAGI-2) (  Nishimura et al., 2002) which binds a variety of postsynaptic molecules including neuroligin, GKAP/SAPAP,  and NMDA receptors as well as presynaptically localized m-Lin 7 (MALS, Velis) (  Perego et al., 2000).	bind
25655	10	6044	5	NULL	NULL	0	NULL	NMDA receptor	NULL		is a type of	NULL				postsynaptic molecule	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellneurosci_27_4_509_s_164	15555928	-catenin also binds to the scaffolding protein S-SCAM (MAGI-2) (  Nishimura et al., 2002) which binds a variety of postsynaptic molecules including neuroligin, GKAP/SAPAP,  and NMDA receptors as well as presynaptically localized m-Lin 7 (MALS, Velis) (  Perego et al., 2000).	bind
18691	1	6044	7	NULL	NULL	NULL	NULL	catenin	GP		bind					S-SCAM	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_27_4_509_s_164	15555928	-catenin also binds to the scaffolding protein S-SCAM (MAGI-2) (  Nishimura et al., 2002) which binds a variety of postsynaptic molecules including neuroligin, GKAP/SAPAP,  and NMDA receptors as well as presynaptically localized m-Lin 7 (MALS, Velis) (  Perego et al., 2000).	bind
18692	2	6044	7	NULL	NULL	NULL	NULL	S-SCAM	GP		bind					neuroligin	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_27_4_509_s_164	15555928	-catenin also binds to the scaffolding protein S-SCAM (MAGI-2) (  Nishimura et al., 2002) which binds a variety of postsynaptic molecules including neuroligin, GKAP/SAPAP,  and NMDA receptors as well as presynaptically localized m-Lin 7 (MALS, Velis) (  Perego et al., 2000).	bind
18693	3	6044	7	NULL	NULL	NULL	NULL	S-SCAM	GP		bind					GKAP/SAPAP	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_27_4_509_s_164	15555928	-catenin also binds to the scaffolding protein S-SCAM (MAGI-2) (  Nishimura et al., 2002) which binds a variety of postsynaptic molecules including neuroligin, GKAP/SAPAP,  and NMDA receptors as well as presynaptically localized m-Lin 7 (MALS, Velis) (  Perego et al., 2000).	bind
18694	4	6044	7	NULL	NULL	NULL	NULL	S-SCAM	GP		bind					NMDA receptors	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_27_4_509_s_164	15555928	-catenin also binds to the scaffolding protein S-SCAM (MAGI-2) (  Nishimura et al., 2002) which binds a variety of postsynaptic molecules including neuroligin, GKAP/SAPAP,  and NMDA receptors as well as presynaptically localized m-Lin 7 (MALS, Velis) (  Perego et al., 2000).	bind
18695	5	6044	7	NULL	NULL	NULL	NULL	S-SCAM	GP		is a type of					scaffolding protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_27_4_509_s_164	15555928	-catenin also binds to the scaffolding protein S-SCAM (MAGI-2) (  Nishimura et al., 2002) which binds a variety of postsynaptic molecules including neuroligin, GKAP/SAPAP,  and NMDA receptors as well as presynaptically localized m-Lin 7 (MALS, Velis) (  Perego et al., 2000).	bind
18696	6	6044	7	NULL	NULL	NULL	NULL	neuroligin	GP		is a type of					postsynaptic molecule	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_27_4_509_s_164	15555928	-catenin also binds to the scaffolding protein S-SCAM (MAGI-2) (  Nishimura et al., 2002) which binds a variety of postsynaptic molecules including neuroligin, GKAP/SAPAP,  and NMDA receptors as well as presynaptically localized m-Lin 7 (MALS, Velis) (  Perego et al., 2000).	bind
18697	7	6044	7	NULL	NULL	NULL	NULL	GKAP/SAPAP	GP		is a type of					postsynaptic molecule	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_27_4_509_s_164	15555928	-catenin also binds to the scaffolding protein S-SCAM (MAGI-2) (  Nishimura et al., 2002) which binds a variety of postsynaptic molecules including neuroligin, GKAP/SAPAP,  and NMDA receptors as well as presynaptically localized m-Lin 7 (MALS, Velis) (  Perego et al., 2000).	bind
18698	8	6044	7	NULL	NULL	NULL	NULL	NMDA receptor 	GP		is a type of					postsynaptic molecule	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_27_4_509_s_164	15555928	-catenin also binds to the scaffolding protein S-SCAM (MAGI-2) (  Nishimura et al., 2002) which binds a variety of postsynaptic molecules including neuroligin, GKAP/SAPAP,  and NMDA receptors as well as presynaptically localized m-Lin 7 (MALS, Velis) (  Perego et al., 2000).	bind
18699	9	6044	7	NULL	NULL	NULL	NULL	S-SCAM	GP		binds					m-Lin 7	GP	presynaptically localized 			NULL		NULL	NULL	NULL	NULL	gw70_molcellneurosci_27_4_509_s_164	15555928	-catenin also binds to the scaffolding protein S-SCAM (MAGI-2) (  Nishimura et al., 2002) which binds a variety of postsynaptic molecules including neuroligin, GKAP/SAPAP,  and NMDA receptors as well as presynaptically localized m-Lin 7 (MALS, Velis) (  Perego et al., 2000).	bind
15743	1	6045	5	NULL	NULL	0	NULL	catenin	NULL		bind	NULL				neurogenin 1	NULL			promoter	NULL	in neural progenitor cells	0	NULL	NULL	NULL	gw70_devbiol_268_1_220_s_202	15031118	-catenin and Lef1 bind to the neurogenin 1 promoter in neural progenitor  cells.	bind
15744	2	6045	5	NULL	NULL	0	NULL	Lef1	NULL		bind	NULL				neurogenin 1	NULL			promoter	NULL	in neural progenitor cells	0	NULL	NULL	NULL	gw70_devbiol_268_1_220_s_202	15031118	-catenin and Lef1 bind to the neurogenin 1 promoter in neural progenitor  cells.	bind
18700	1	6045	7	NULL	NULL	NULL	NULL	catenin	GP		binds to					neurogenin 1	GP			promoter	NULL	neural progenitor cells	NULL	NULL	NULL	NULL	gw70_devbiol_268_1_220_s_202	15031118	-catenin and Lef1 bind to the neurogenin 1 promoter in neural progenitor  cells.	bind
18701	2	6045	7	NULL	NULL	NULL	NULL	Lef1 	GP		binds to					neurogenin 1	GP			promoter	NULL	neural progenitor cells	NULL	NULL	NULL	NULL	gw70_devbiol_268_1_220_s_202	15031118	-catenin and Lef1 bind to the neurogenin 1 promoter in neural progenitor  cells.	bind
15745	1	6046	5	NULL	NULL	0	NULL	Catenin	NULL		associate with	NULL				cadherin	NULL		cytoplasmic domain		NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1495_2_168_s_58	10656974	-Catenin associates with the cytoplasmic domain of cadherins [  16], and binds the vinculin-related protein  -catenin, which in turn makes contact to actin filaments [  17].	bind
15746	2	6046	5	NULL	NULL	0	NULL	Catenin	NULL		bind	NULL				catenin	NULL	vinculin-related protein			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1495_2_168_s_58	10656974	-Catenin associates with the cytoplasmic domain of cadherins [  16], and binds the vinculin-related protein  -catenin, which in turn makes contact to actin filaments [  17].	bind
15747	3	6046	5	NULL	NULL	0	NULL	catenin	NULL		makes contact to	NULL				actin filaments	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1495_2_168_s_58	10656974	-Catenin associates with the cytoplasmic domain of cadherins [  16], and binds the vinculin-related protein  -catenin, which in turn makes contact to actin filaments [  17].	bind
25656	4	6046	5	NULL	NULL	0	NULL	catenin	NULL		is a type of	NULL				vinculin-related protein	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1495_2_168_s_58	10656974	-Catenin associates with the cytoplasmic domain of cadherins [  16], and binds the vinculin-related protein  -catenin, which in turn makes contact to actin filaments [  17].	bind
18702	1	6046	7	NULL	NULL	NULL	NULL	Catenin	GP		associate with					cadherins	GP		cytoplasmic domain		NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1495_2_168_s_58	10656974	-Catenin associates with the cytoplasmic domain of cadherins [  16], and binds the vinculin-related protein  -catenin, which in turn makes contact to actin filaments [  17].	bind
18703	2	6046	7	NULL	NULL	NULL	NULL	statement 1	Process		bind					catenin	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1495_2_168_s_58	10656974	-Catenin associates with the cytoplasmic domain of cadherins [  16], and binds the vinculin-related protein  -catenin, which in turn makes contact to actin filaments [  17].	bind
18704	3	6046	7	NULL	NULL	NULL	NULL	statement 2	Process		makes contact to					actin filaments	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1495_2_168_s_58	10656974	-Catenin associates with the cytoplasmic domain of cadherins [  16], and binds the vinculin-related protein  -catenin, which in turn makes contact to actin filaments [  17].	bind
25644	4	6046	7	NULL	NULL	NULL	NULL	catenin	GP		is a type of					vinculin related protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1495_2_168_s_58	10656974	-Catenin associates with the cytoplasmic domain of cadherins [  16], and binds the vinculin-related protein  -catenin, which in turn makes contact to actin filaments [  17].	bind
15748	1	6047	5	10	NULL	0	NULL	catenin			bind			armadillo repeats		cadherin			cytoplasmic tail 		NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_13_0_119_s_151	9442870	-catenin binds to the cadherin cytoplasmic tail via its centrally located armadillo  repeats ( Hulsken et al 1994,  Funayama et al 1995), 40 amino acid protein-protein-binding motifs originally described in the  Drosophila homologue of  -catenin Armadillo ( Peifer & Wieschaus 1990,  Peifer et al 1994).	bind
54142	2	6047	5	10	NULL	0	NULL	catenin			is located			armadillo repeats		centrally					NULL		0	NULL	NULL	NULL	gw70_annurevcelldevbiol_13_0_119_s_151	9442870	-catenin binds to the cadherin cytoplasmic tail via its centrally located armadillo  repeats ( Hulsken et al 1994,  Funayama et al 1995), 40 amino acid protein-protein-binding motifs originally described in the  Drosophila homologue of  -catenin Armadillo ( Peifer & Wieschaus 1990,  Peifer et al 1994).	bind
18705	1	6047	7	NULL	NULL	NULL	NULL	catenin 	GP		bind			armadillo repeats		cadherin	GP		cytoplasmic tail		NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_13_0_119_s_151	9442870	-catenin binds to the cadherin cytoplasmic tail via its centrally located armadillo  repeats ( Hulsken et al 1994,  Funayama et al 1995), 40 amino acid protein-protein-binding motifs originally described in the  Drosophila homologue of  -catenin Armadillo ( Peifer & Wieschaus 1990,  Peifer et al 1994).	bind
18706	2	6047	7	NULL	NULL	NULL	NULL	catenin	GP		is located			armadillo repeats		centrally	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_13_0_119_s_151	9442870	-catenin binds to the cadherin cytoplasmic tail via its centrally located armadillo  repeats ( Hulsken et al 1994,  Funayama et al 1995), 40 amino acid protein-protein-binding motifs originally described in the  Drosophila homologue of  -catenin Armadillo ( Peifer & Wieschaus 1990,  Peifer et al 1994).	bind
18707	3	6047	7	NULL	NULL	NULL	NULL	armadillo repeats	GP		is					catenin Armadillo	GP	Drosophila homologue of 	40 amino acid protein-protein-binding motifs		NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_13_0_119_s_151	9442870	-catenin binds to the cadherin cytoplasmic tail via its centrally located armadillo  repeats ( Hulsken et al 1994,  Funayama et al 1995), 40 amino acid protein-protein-binding motifs originally described in the  Drosophila homologue of  -catenin Armadillo ( Peifer & Wieschaus 1990,  Peifer et al 1994).	bind
15749	1	6048	5	NULL	NULL	0	NULL	transcription factors	NULL		bind	NULL				AP-1 complex	NULL				NULL		0	NULL	NULL	NULL	gw60_neuroscience_108_3_371_s_166	11738252	-Catenin could also play a role in increasing Cdk5 expression because of its ability to increase transcription factors which bind to the AP-1 complex.	bind
15750	2	6048	5	NULL	NULL	0	NULL	Catenin	NULL		increase	NULL				transcription factors	NULL				NULL		0	NULL	NULL	NULL	gw60_neuroscience_108_3_371_s_166	11738252	-Catenin could also play a role in increasing Cdk5 expression because of its ability to increase transcription factors which bind to the AP-1 complex.	bind
15751	3	6048	5	10	NULL	0	NULL	Catenin			increase					Catenin		expression of			NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_108_3_371_s_166	11738252	-Catenin could also play a role in increasing Cdk5 expression because of its ability to increase transcription factors which bind to the AP-1 complex.	bind
15752	4	6048	5	NULL	NULL	0	NULL	statement 3	NULL		because of	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_neuroscience_108_3_371_s_166	11738252	-Catenin could also play a role in increasing Cdk5 expression because of its ability to increase transcription factors which bind to the AP-1 complex.	bind
18745	1	6048	7	NULL	NULL	NULL	NULL	Catenin	GP		increase					Cdk5	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_108_3_371_s_166	11738252	-Catenin could also play a role in increasing Cdk5 expression because of its ability to increase transcription factors which bind to the AP-1 complex.	bind
18746	2	6048	7	NULL	NULL	NULL	NULL	Catenin	GP		increase					transcription factors	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_108_3_371_s_166	11738252	-Catenin could also play a role in increasing Cdk5 expression because of its ability to increase transcription factors which bind to the AP-1 complex.	bind
18747	3	6048	7	NULL	NULL	NULL	NULL	transcription factors	GP		bind					AP-1 complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_108_3_371_s_166	11738252	-Catenin could also play a role in increasing Cdk5 expression because of its ability to increase transcription factors which bind to the AP-1 complex.	bind
15753	1	6049	5	NULL	NULL	0	NULL	Crystallin	NULL		bind	NULL				alphaA-crystallin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_18_10449_s_72	8631839	-Crystallin  bound to alphaA-crystallin shows an emission maximum at 337 nm,  i.e.  red-shifted only by 7 nm from that of its native state.	bind
18748	1	6049	7	NULL	NULL	NULL	NULL	Crystallin	GP		bind					alphaA-crystallin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_18_10449_s_72	8631839	-Crystallin  bound to alphaA-crystallin shows an emission maximum at 337 nm,  i.e.  red-shifted only by 7 nm from that of its native state.	bind
15754	1	6050	5	NULL	NULL	0	NULL	Crystallin	NULL		bind	NULL	specifically			NADP(H)	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26224_s_235	7592828	-Crystallin  specifically binds NADP(H) and is a novel NADPH:quinone  oxidoreductase( 35,  49) .	bind
15755	2	6050	5	NULL	NULL	0	NULL	Crystallin	NULL		is	NULL				NADPH:quinone oxidoreductase	NULL	novel			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26224_s_235	7592828	-Crystallin  specifically binds NADP(H) and is a novel NADPH:quinone  oxidoreductase( 35,  49) .	bind
18844	1	6050	7	NULL	NULL	NULL	NULL	Crystallin	GP		binds		specifically			NADP(H)	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_44_26224_s_235	7592828	-Crystallin  specifically binds NADP(H) and is a novel NADPH:quinone  oxidoreductase( 35,  49) .	bind
18845	2	6050	7	NULL	NULL	NULL	NULL	Crystallin	GP		is a type of					NADPH:quinone oxidoreductase	GP	novel			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_44_26224_s_235	7592828	-Crystallin  specifically binds NADP(H) and is a novel NADPH:quinone  oxidoreductase( 35,  49) .	bind
15756	1	6052	5	NULL	NULL	0	NULL	Crystallin	NULL		bind	NULL				MDA	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1500_1_49_s_174	10564717	-Crystallin itself binds MDA, resulting in a fluorescent adduct.	bind
18846	1	6052	7	NULL	NULL	NULL	NULL	Crystallin	GP		binds					MDA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1500_1_49_s_174	10564717	-Crystallin itself binds MDA, resulting in a fluorescent adduct.	bind
18847	2	6052	7	NULL	NULL	NULL	NULL	statement 1	Process		results in					fluorescent adduct	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1500_1_49_s_174	10564717	-Crystallin itself binds MDA, resulting in a fluorescent adduct.	bind
15757	1	6053	5	NULL	NULL	0	NULL	agrin	NULL		bind	NULL				DG	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_4_5_783_s_41	10619025	-DG binding by agrin may contribute to this process but has additional important functions in nonmuscle tissues (  Yamada et al. 1996a  ; Gesemann et al. 1998  ).	bind
18848	1	6053	7	NULL	NULL	NULL	NULL	agrin	GP		binds					DG	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_4_5_783_s_41	10619025	-DG binding by agrin may contribute to this process but has additional important functions in nonmuscle tissues (  Yamada et al. 1996a  ; Gesemann et al. 1998  ).	bind
15758	1	6054	5	NULL	NULL	0	NULL	agrin	NULL		interacts with	NULL				dystrophin	NULL				NULL	inside cytoplasm	0	NULL	NULL	NULL	gw60_febslett_499_3_210_s_8	11423118	-DG, which contains the transmembrane domain, interacts with dystrophin and dystrophin-related proteins inside the cytoplasm, whereas  -DG, the highly glycosylated peripheral membrane subunit, binds extracellular matrix proteins containing laminin-type LG domains [  6,   7 and   8].	bind
15759	2	6054	5	NULL	NULL	0	NULL	DG	NULL		interacts with	NULL				dystrophin-related proteins	NULL				NULL	inside cytoplasm	0	NULL	NULL	NULL	gw60_febslett_499_3_210_s_8	11423118	-DG, which contains the transmembrane domain, interacts with dystrophin and dystrophin-related proteins inside the cytoplasm, whereas  -DG, the highly glycosylated peripheral membrane subunit, binds extracellular matrix proteins containing laminin-type LG domains [  6,   7 and   8].	bind
15760	3	6054	5	10	NULL	0	NULL	DG			bind					statement 5					NULL		NULL	NULL	NULL	NULL	gw60_febslett_499_3_210_s_8	11423118	-DG, which contains the transmembrane domain, interacts with dystrophin and dystrophin-related proteins inside the cytoplasm, whereas  -DG, the highly glycosylated peripheral membrane subunit, binds extracellular matrix proteins containing laminin-type LG domains [  6,   7 and   8].	bind
25658	4	6054	5	10	NULL	0	NULL	DG			is a type of							highly glycosylated	peripheral membrane subunit		NULL		NULL	NULL	NULL	NULL	gw60_febslett_499_3_210_s_8	11423118	-DG, which contains the transmembrane domain, interacts with dystrophin and dystrophin-related proteins inside the cytoplasm, whereas  -DG, the highly glycosylated peripheral membrane subunit, binds extracellular matrix proteins containing laminin-type LG domains [  6,   7 and   8].	bind
54146	5	6054	5	10	NULL	0	NULL	extracellular matrix proteins			contains								laminin-type LG domains		NULL		0	NULL	NULL	NULL	gw60_febslett_499_3_210_s_8	11423118	-DG, which contains the transmembrane domain, interacts with dystrophin and dystrophin-related proteins inside the cytoplasm, whereas  -DG, the highly glycosylated peripheral membrane subunit, binds extracellular matrix proteins containing laminin-type LG domains [  6,   7 and   8].	bind
18849	1	6054	7	NULL	NULL	NULL	NULL	DG	GP		contains								transmembrane domain		NULL		NULL	NULL	NULL	NULL	gw60_febslett_499_3_210_s_8	11423118	-DG, which contains the transmembrane domain, interacts with dystrophin and dystrophin-related proteins inside the cytoplasm, whereas  -DG, the highly glycosylated peripheral membrane subunit, binds extracellular matrix proteins containing laminin-type LG domains [  6,   7 and   8].	bind
18850	2	6054	7	NULL	NULL	NULL	NULL	statement 1	Process		interacts with					dystrophin	GP				NULL	inside cytoplasm \t	NULL	NULL	NULL	NULL	gw60_febslett_499_3_210_s_8	11423118	-DG, which contains the transmembrane domain, interacts with dystrophin and dystrophin-related proteins inside the cytoplasm, whereas  -DG, the highly glycosylated peripheral membrane subunit, binds extracellular matrix proteins containing laminin-type LG domains [  6,   7 and   8].	bind
18851	3	6054	7	NULL	NULL	NULL	NULL	statement 1	Process		interacts with					 dystrophin-related proteins	GP				NULL	inside the cytoplasm	NULL	NULL	NULL	NULL	gw60_febslett_499_3_210_s_8	11423118	-DG, which contains the transmembrane domain, interacts with dystrophin and dystrophin-related proteins inside the cytoplasm, whereas  -DG, the highly glycosylated peripheral membrane subunit, binds extracellular matrix proteins containing laminin-type LG domains [  6,   7 and   8].	bind
18852	4	6054	7	NULL	NULL	NULL	NULL	DG	GP		is a type of							highly glycosylated	peripheral membrane subunit		NULL		NULL	NULL	NULL	NULL	gw60_febslett_499_3_210_s_8	11423118	-DG, which contains the transmembrane domain, interacts with dystrophin and dystrophin-related proteins inside the cytoplasm, whereas  -DG, the highly glycosylated peripheral membrane subunit, binds extracellular matrix proteins containing laminin-type LG domains [  6,   7 and   8].	bind
18853	5	6054	7	NULL	NULL	NULL	NULL	DG	GP		binds					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_499_3_210_s_8	11423118	-DG, which contains the transmembrane domain, interacts with dystrophin and dystrophin-related proteins inside the cytoplasm, whereas  -DG, the highly glycosylated peripheral membrane subunit, binds extracellular matrix proteins containing laminin-type LG domains [  6,   7 and   8].	bind
54147	6	6054	7	NULL	NULL	NULL	NULL	extracellular matrix protein	GP		contains								laminin-type LG domains		NULL		NULL	NULL	NULL	NULL	gw60_febslett_499_3_210_s_8	11423118	-DG, which contains the transmembrane domain, interacts with dystrophin and dystrophin-related proteins inside the cytoplasm, whereas  -DG, the highly glycosylated peripheral membrane subunit, binds extracellular matrix proteins containing laminin-type LG domains [  6,   7 and   8].	bind
15761	1	6055	5	NULL	NULL	0	NULL	Dystroglycan	NULL		bind	NULL				laminin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_20_11711_s_10	7744812	-Dystroglycan binds laminin and dystrophin binds actin filaments,  indicating that one function of the dystrophin-glycoprotein complex is  to provide a link between the extracellular matrix and the cell  cytoskeleton ( 5,  6) .	bind
15762	2	6055	5	NULL	NULL	0	NULL	dystrophin	NULL		bind	NULL				actin filaments	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_20_11711_s_10	7744812	-Dystroglycan binds laminin and dystrophin binds actin filaments,  indicating that one function of the dystrophin-glycoprotein complex is  to provide a link between the extracellular matrix and the cell  cytoskeleton ( 5,  6) .	bind
15763	4	6055	5	NULL	NULL	0	NULL	dystrophin-glycoprotein complex	NULL		plays a role in	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_20_11711_s_10	7744812	-Dystroglycan binds laminin and dystrophin binds actin filaments,  indicating that one function of the dystrophin-glycoprotein complex is  to provide a link between the extracellular matrix and the cell  cytoskeleton ( 5,  6) .	bind
45614	3	6055	5	NULL	NULL	0	NULL	extracellular matrix	NULL		is linked to	NULL				cell cytoskeleton	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_20_11711_s_10	7744812	-Dystroglycan binds laminin and dystrophin binds actin filaments,  indicating that one function of the dystrophin-glycoprotein complex is  to provide a link between the extracellular matrix and the cell  cytoskeleton ( 5,  6) .	bind
18855	1	6055	7	NULL	NULL	NULL	NULL	Dystroglycan	GP		binds					laminin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_20_11711_s_10	7744812	-Dystroglycan binds laminin and dystrophin binds actin filaments,  indicating that one function of the dystrophin-glycoprotein complex is  to provide a link between the extracellular matrix and the cell  cytoskeleton ( 5,  6) .	bind
18856	2	6055	7	NULL	NULL	NULL	NULL	dystrophin	GP		binds					actin filaments	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_20_11711_s_10	7744812	-Dystroglycan binds laminin and dystrophin binds actin filaments,  indicating that one function of the dystrophin-glycoprotein complex is  to provide a link between the extracellular matrix and the cell  cytoskeleton ( 5,  6) .	bind
18857	3	6055	7	NULL	NULL	NULL	NULL	extracellular matrix	CellComponent		is linked to					cell cytoskeleton	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_20_11711_s_10	7744812	-Dystroglycan binds laminin and dystrophin binds actin filaments,  indicating that one function of the dystrophin-glycoprotein complex is  to provide a link between the extracellular matrix and the cell  cytoskeleton ( 5,  6) .	bind
44932	4	6055	7	NULL	NULL	NULL	NULL	dystrophin-glycoprotein complex	GP		plays a role in					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_20_11711_s_10	7744812	-Dystroglycan binds laminin and dystrophin binds actin filaments,  indicating that one function of the dystrophin-glycoprotein complex is  to provide a link between the extracellular matrix and the cell  cytoskeleton ( 5,  6) .	bind
15764	1	6056	5	10	NULL	0	NULL	Dystroglycan	NULL		bind	NULL				dystrophin	NULL		cysteine-rich C-terminal domain		NULL		NULL	NULL	NULL	NULL	gw70_annurevmed_48_0_457_s_52	9046976	-Dystroglycan binds to the cysteine-rich region of the  C-terminal domain of dystrophin ( 15,  18).	bind
18858	1	6056	7	NULL	NULL	NULL	NULL	Dystroglycan	GP		binds to					dystrophin	GP		cysteine-rich  C-terminal domain		NULL		NULL	NULL	NULL	NULL	gw70_annurevmed_48_0_457_s_52	9046976	-Dystroglycan binds to the cysteine-rich region of the  C-terminal domain of dystrophin ( 15,  18).	bind
15765	1	6057	5	10	NULL	0	NULL	Dystroglycan	NULL		bind	NULL				dystrophin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1573_3_292_s_146	12417411	-Dystroglycan is a transmembrane protein which binds dystrophin and the intracellular cytoskeleton.	bind
15766	2	6057	5	10	NULL	0	NULL	Dystroglycan	NULL		bind	NULL				cytoskeleton	NULL	intracellular			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1573_3_292_s_146	12417411	-Dystroglycan is a transmembrane protein which binds dystrophin and the intracellular cytoskeleton.	bind
44842	3	6057	5	10	NULL	0	NULL	Dystroglycan	NULL		is a type of	NULL				transmembrane protein	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1573_3_292_s_146	12417411	-Dystroglycan is a transmembrane protein which binds dystrophin and the intracellular cytoskeleton.	bind
18859	1	6057	7	NULL	NULL	NULL	NULL	Dystroglycan	GP		binds					dystrophin	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1573_3_292_s_146	12417411	-Dystroglycan is a transmembrane protein which binds dystrophin and the intracellular cytoskeleton.	bind
18860	2	6057	7	NULL	NULL	NULL	NULL	Dystroglycan	GP		binds					cytoskeleton	CellComponent	intracellular			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1573_3_292_s_146	12417411	-Dystroglycan is a transmembrane protein which binds dystrophin and the intracellular cytoskeleton.	bind
44843	3	6057	7	NULL	NULL	NULL	NULL	Dystroglycan	GP		is a type of					transmembrane protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1573_3_292_s_146	12417411	-Dystroglycan is a transmembrane protein which binds dystrophin and the intracellular cytoskeleton.	bind
15767	1	6058	5	NULL	NULL	0	NULL	Glutamate uptake inhibitors	NULL		stimulate	NULL				phosphoinositide 	NULL	hydrolysis of			NULL	in baby hamster kidney cells expressing mGluR1a	0	NULL	NULL	NULL	gw60_neuropharmacology_37_12_1465_s_319	9886669	-Glutamate uptake inhibitors may stimulate phosphoinositide hydrolysis in baby hamster kidney cells expressing mGluR1a via heteroexchange with  -glutamate without direct activation of mGluR1a.	bind
15768	2	6058	5	10	NULL	0	NULL	statement 1			occurs via					glutamate		heteroexchange with 			NULL	baby hamster kidney cells expressing mGluR1a	NULL	NULL	NULL	NULL	gw60_neuropharmacology_37_12_1465_s_319	9886669	-Glutamate uptake inhibitors may stimulate phosphoinositide hydrolysis in baby hamster kidney cells expressing mGluR1a via heteroexchange with  -glutamate without direct activation of mGluR1a.	bind
15769	3	6058	5	10	NULL	0	NULL	statement 2			occurs without					mGluR1a		activation of			NULL	baby hamster kidney cells expressing mGluR1a	NULL	NULL	NULL	NULL	gw60_neuropharmacology_37_12_1465_s_319	9886669	-Glutamate uptake inhibitors may stimulate phosphoinositide hydrolysis in baby hamster kidney cells expressing mGluR1a via heteroexchange with  -glutamate without direct activation of mGluR1a.	bind
18876	1	6058	7	NULL	NULL	NULL	NULL	Glutamate uptake inhibitors	Chemical		stimulate		may			phosphoinositide	Chemical	hydrolysis of			NULL	baby hamster kidney cells expressing mGluR1a	NULL	NULL	NULL	NULL	gw60_neuropharmacology_37_12_1465_s_319	9886669	-Glutamate uptake inhibitors may stimulate phosphoinositide hydrolysis in baby hamster kidney cells expressing mGluR1a via heteroexchange with  -glutamate without direct activation of mGluR1a.	bind
18878	2	6058	7	NULL	NULL	NULL	NULL	statement 2	Process		occurs via					glutamate	AminoAcid	heteroexchange with			NULL	baby hamster kidney cells expressing mGluR1a	NULL	NULL	NULL	NULL	gw60_neuropharmacology_37_12_1465_s_319	9886669	-Glutamate uptake inhibitors may stimulate phosphoinositide hydrolysis in baby hamster kidney cells expressing mGluR1a via heteroexchange with  -glutamate without direct activation of mGluR1a.	bind
18881	3	6058	7	NULL	NULL	NULL	NULL	statement 2	Process		happens without					mGluR1a	GP	direct activation of 			NULL	baby hamster kidney cells expressing mGluR1a	NULL	NULL	NULL	NULL	gw60_neuropharmacology_37_12_1465_s_319	9886669	-Glutamate uptake inhibitors may stimulate phosphoinositide hydrolysis in baby hamster kidney cells expressing mGluR1a via heteroexchange with  -glutamate without direct activation of mGluR1a.	bind
15770	1	6059	5	NULL	NULL	0	NULL	cisplatin	NULL		bind	NULL				GSH	NULL				NULL		0	NULL	NULL	NULL	gw70_intjdevneurosci_18_2_259_s_133	10715580	-Met and  -Met, free radical scavengers, may act by several different mechanisms including direct  binding to cisplatin itself or by reversing the binding of cisplatin to GSH [ 25].	bind
15771	2	6059	5	10	NULL	0	NULL	Met			act by		may			cisplatin		direct binding to			NULL		NULL	NULL	NULL	NULL	gw70_intjdevneurosci_18_2_259_s_133	10715580	-Met and  -Met, free radical scavengers, may act by several different mechanisms including direct  binding to cisplatin itself or by reversing the binding of cisplatin to GSH [ 25].	bind
15772	3	6059	5	10	NULL	0	NULL	Met			act by		may			statement 1		reversing			NULL		NULL	NULL	NULL	NULL	gw70_intjdevneurosci_18_2_259_s_133	10715580	-Met and  -Met, free radical scavengers, may act by several different mechanisms including direct  binding to cisplatin itself or by reversing the binding of cisplatin to GSH [ 25].	bind
15773	4	6059	5	NULL	NULL	0	NULL	Met, free radical scavengers	NULL		act by	NULL	may			cisplatin	NULL	direct binding to			NULL		0	NULL	NULL	NULL	gw70_intjdevneurosci_18_2_259_s_133	10715580	-Met and  -Met, free radical scavengers, may act by several different mechanisms including direct  binding to cisplatin itself or by reversing the binding of cisplatin to GSH [ 25].	bind
15774	5	6059	5	NULL	NULL	0	NULL	Met, free radical scavengers	NULL		act by	NULL	may			statement 1	NULL	reversing			NULL		0	NULL	NULL	NULL	gw70_intjdevneurosci_18_2_259_s_133	10715580	-Met and  -Met, free radical scavengers, may act by several different mechanisms including direct  binding to cisplatin itself or by reversing the binding of cisplatin to GSH [ 25].	bind
18883	1	6059	7	NULL	NULL	NULL	NULL	Met	AminoAcid		bind		directly			cisplatin	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_intjdevneurosci_18_2_259_s_133	10715580	-Met and  -Met, free radical scavengers, may act by several different mechanisms including direct  binding to cisplatin itself or by reversing the binding of cisplatin to GSH [ 25].	bind
18884	2	6059	7	NULL	NULL	NULL	NULL	Met free radical scavengers	Chemical		bind		directly			cisplatin	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_intjdevneurosci_18_2_259_s_133	10715580	-Met and  -Met, free radical scavengers, may act by several different mechanisms including direct  binding to cisplatin itself or by reversing the binding of cisplatin to GSH [ 25].	bind
18887	4	6059	7	NULL	NULL	NULL	NULL	statement 1	Process		reverse					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_intjdevneurosci_18_2_259_s_133	10715580	-Met and  -Met, free radical scavengers, may act by several different mechanisms including direct  binding to cisplatin itself or by reversing the binding of cisplatin to GSH [ 25].	bind
18888	6	6059	7	NULL	NULL	NULL	NULL	statement 2	Process		reverse					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_intjdevneurosci_18_2_259_s_133	10715580	-Met and  -Met, free radical scavengers, may act by several different mechanisms including direct  binding to cisplatin itself or by reversing the binding of cisplatin to GSH [ 25].	bind
45622	3	6059	7	NULL	NULL	NULL	NULL	cisplatin	Chemical		bind					GSH	GP				NULL		NULL	NULL	NULL	NULL	gw70_intjdevneurosci_18_2_259_s_133	10715580	-Met and  -Met, free radical scavengers, may act by several different mechanisms including direct  binding to cisplatin itself or by reversing the binding of cisplatin to GSH [ 25].	bind
15775	1	6060	5	NULL	NULL	0	NULL	MSH	NULL		bind	NULL				MC1R	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevgenet_38_0_365_s_336	15568981	-MSH binds MC1R and induces the activation of the  S-coupled G protein, which  then activates adenylyl cyclase.	bind
15776	2	6060	5	10	NULL	0	NULL	statement 1			induce					S-coupled G protein		activation of			NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_38_0_365_s_336	15568981	-MSH binds MC1R and induces the activation of the  S-coupled G protein, which  then activates adenylyl cyclase.	bind
15777	3	6060	5	NULL	NULL	0	NULL	statement 2	NULL		activate	NULL				S-coupled G protein	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevgenet_38_0_365_s_336	15568981	-MSH binds MC1R and induces the activation of the  S-coupled G protein, which  then activates adenylyl cyclase.	bind
18889	1	6060	7	NULL	NULL	NULL	NULL	MSH	GP		binds					MC1R	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_38_0_365_s_336	15568981	-MSH binds MC1R and induces the activation of the  S-coupled G protein, which  then activates adenylyl cyclase.	bind
18890	2	6060	7	NULL	NULL	NULL	NULL	statement 1	Process		induce					S-coupled G protein	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_38_0_365_s_336	15568981	-MSH binds MC1R and induces the activation of the  S-coupled G protein, which  then activates adenylyl cyclase.	bind
18891	3	6060	7	NULL	NULL	NULL	NULL	statement 2	Process		activates					adenylyl cyclase	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_38_0_365_s_336	15568981	-MSH binds MC1R and induces the activation of the  S-coupled G protein, which  then activates adenylyl cyclase.	bind
15828	1	6061	5	NULL	NULL	0	NULL	MSH	NULL		bind	NULL	predominantly			receptor MC-1R	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_549_1_87_s_277	12914931	-MSH binds predominantly with its receptor MC-1R.	bind
18892	1	6061	7	NULL	NULL	NULL	NULL	MSH	GP		binds		predominantly			MC-1R receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_549_1_87_s_277	12914931	-MSH binds predominantly with its receptor MC-1R.	bind
15829	1	6062	5	NULL	NULL	0	NULL	MSH	NULL		is a type of	NULL				cell surface receptor	NULL				NULL		NULL	NULL	NULL	NULL	gw60_febslett_549_1_87_s_151	12914931	-MSH binds with its cell surface receptor specifically melanocortin-1 receptor (MC-1R).	bind
15830	2	6062	5	NULL	NULL	0	NULL	MSH	NULL		bind	NULL	specifically			MC-1R	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_549_1_87_s_151	12914931	-MSH binds with its cell surface receptor specifically melanocortin-1 receptor (MC-1R).	bind
15831	3	6062	5	NULL	NULL	0	NULL	MC-1R	NULL		is	NULL				melanocortin-1 receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_549_1_87_s_151	12914931	-MSH binds with its cell surface receptor specifically melanocortin-1 receptor (MC-1R).	bind
18893	1	6062	7	NULL	NULL	NULL	NULL	MSH	GP		binds		specifically			MC-1R	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_549_1_87_s_151	12914931	-MSH binds with its cell surface receptor specifically melanocortin-1 receptor (MC-1R).	bind
18894	2	6062	7	NULL	NULL	NULL	NULL	MC-1R	GP		is					melanocortin-1 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_549_1_87_s_151	12914931	-MSH binds with its cell surface receptor specifically melanocortin-1 receptor (MC-1R).	bind
25657	3	6062	7	NULL	NULL	NULL	NULL	MC-1R	GP		is a type of					cell surface receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_549_1_87_s_151	12914931	-MSH binds with its cell surface receptor specifically melanocortin-1 receptor (MC-1R).	bind
15854	1	6063	5	NULL	NULL	0	NULL	BTX	NULL		bind	NULL	specifically			AChR	NULL				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_2_147_s_22	11251289	-Neurotoxins such as  -bungarotoxin ( -BTX) bind specifically to AChR and exhibit high toxicity due to inhibition of the AChR function at the neuromuscular junction.	bind
15855	2	6063	5	NULL	NULL	0	NULL	BTX	NULL		is	NULL				bungarotoxin	NULL				NULL		0	NULL	NULL	NULL	gw60_chembiol_8_2_147_s_22	11251289	-Neurotoxins such as  -bungarotoxin ( -BTX) bind specifically to AChR and exhibit high toxicity due to inhibition of the AChR function at the neuromuscular junction.	bind
15856	3	6063	5	NULL	NULL	0	NULL	BTX	NULL		exhibit	NULL				toxicity 	NULL	high			NULL	at neuromuscular junction	0	NULL	NULL	NULL	gw60_chembiol_8_2_147_s_22	11251289	-Neurotoxins such as  -bungarotoxin ( -BTX) bind specifically to AChR and exhibit high toxicity due to inhibition of the AChR function at the neuromuscular junction.	bind
15858	4	6063	5	10	NULL	0	NULL	statement 3	NULL		occurs due to	NULL				AChR	NULL	inhibition of;; function of			NULL	at neuromuscular junction	NULL	NULL	NULL	NULL	gw60_chembiol_8_2_147_s_22	11251289	-Neurotoxins such as  -bungarotoxin ( -BTX) bind specifically to AChR and exhibit high toxicity due to inhibition of the AChR function at the neuromuscular junction.	bind
25659	5	6063	5	NULL	NULL	0	NULL	BTX	NULL		is a type of	NULL				neurotoxin	NULL				NULL		0	NULL	NULL	NULL	gw60_chembiol_8_2_147_s_22	11251289	-Neurotoxins such as  -bungarotoxin ( -BTX) bind specifically to AChR and exhibit high toxicity due to inhibition of the AChR function at the neuromuscular junction.	bind
18895	1	6063	7	NULL	NULL	NULL	NULL	BTX	GP		bind		specifically			AChR	GP				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_2_147_s_22	11251289	-Neurotoxins such as  -bungarotoxin ( -BTX) bind specifically to AChR and exhibit high toxicity due to inhibition of the AChR function at the neuromuscular junction.	bind
18896	2	6063	7	NULL	NULL	NULL	NULL	BTX	GP		possess					high toxicity	Process				NULL	neuromuscular junction	NULL	NULL	NULL	NULL	gw60_chembiol_8_2_147_s_22	11251289	-Neurotoxins such as  -bungarotoxin ( -BTX) bind specifically to AChR and exhibit high toxicity due to inhibition of the AChR function at the neuromuscular junction.	bind
18897	3	6063	7	NULL	NULL	NULL	NULL	statement 2	Process		occurs due to					AChR	GP	inhibition of;; function of			NULL	neuromuscular junction	NULL	NULL	NULL	NULL	gw60_chembiol_8_2_147_s_22	11251289	-Neurotoxins such as  -bungarotoxin ( -BTX) bind specifically to AChR and exhibit high toxicity due to inhibition of the AChR function at the neuromuscular junction.	bind
18899	5	6063	7	NULL	NULL	NULL	NULL	BTX	GP		is					bungarotoxin	GP				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_2_147_s_22	11251289	-Neurotoxins such as  -bungarotoxin ( -BTX) bind specifically to AChR and exhibit high toxicity due to inhibition of the AChR function at the neuromuscular junction.	bind
18900	6	6063	7	NULL	NULL	NULL	NULL	bungarotoxin	GP		is a type of					neurotoxin	GP				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_2_147_s_22	11251289	-Neurotoxins such as  -bungarotoxin ( -BTX) bind specifically to AChR and exhibit high toxicity due to inhibition of the AChR function at the neuromuscular junction.	bind
15859	1	6064	5	NULL	NULL	0	NULL	Pak2	NULL		is	NULL				PAK	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_515_1_84_s_3	11943200	-PAK (Pak2) is a ubiquitous member of the family of p21-activated protein kinases (PAKs) which are activated by autophosphorylation following binding of the GTP-bound form of the small G-protein Cdc42 (for reviews see [  1,   2,   3,   4 and   5]).	bind
15860	2	6064	5	NULL	NULL	0	NULL	Pak2	NULL		is a type of	NULL				p21-activated protein kinases	NULL				NULL		NULL	NULL	NULL	NULL	gw60_febslett_515_1_84_s_3	11943200	-PAK (Pak2) is a ubiquitous member of the family of p21-activated protein kinases (PAKs) which are activated by autophosphorylation following binding of the GTP-bound form of the small G-protein Cdc42 (for reviews see [  1,   2,   3,   4 and   5]).	bind
15861	3	6064	5	NULL	NULL	0	NULL	Pak2	NULL		activated by	NULL				autophosphorylation	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_515_1_84_s_3	11943200	-PAK (Pak2) is a ubiquitous member of the family of p21-activated protein kinases (PAKs) which are activated by autophosphorylation following binding of the GTP-bound form of the small G-protein Cdc42 (for reviews see [  1,   2,   3,   4 and   5]).	bind
15862	4	6064	5	10	NULL	0	NULL	GTP	NULL		bind	NULL				Cdc42	NULL				NULL		NULL	NULL	NULL	NULL	gw60_febslett_515_1_84_s_3	11943200	-PAK (Pak2) is a ubiquitous member of the family of p21-activated protein kinases (PAKs) which are activated by autophosphorylation following binding of the GTP-bound form of the small G-protein Cdc42 (for reviews see [  1,   2,   3,   4 and   5]).	bind
15863	5	6064	5	10	NULL	0	NULL	statement 3	NULL		occurs upon	NULL				statement 4	NULL				NULL		NULL	NULL	NULL	NULL	gw60_febslett_515_1_84_s_3	11943200	-PAK (Pak2) is a ubiquitous member of the family of p21-activated protein kinases (PAKs) which are activated by autophosphorylation following binding of the GTP-bound form of the small G-protein Cdc42 (for reviews see [  1,   2,   3,   4 and   5]).	bind
44844	6	6064	5	10	NULL	0	NULL	Cdc42	NULL		is a type of	NULL				small G protein	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_515_1_84_s_3	11943200	-PAK (Pak2) is a ubiquitous member of the family of p21-activated protein kinases (PAKs) which are activated by autophosphorylation following binding of the GTP-bound form of the small G-protein Cdc42 (for reviews see [  1,   2,   3,   4 and   5]).	bind
18901	1	6064	7	NULL	NULL	NULL	NULL	GTP	Chemical		bind					Cdc42	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_515_1_84_s_3	11943200	-PAK (Pak2) is a ubiquitous member of the family of p21-activated protein kinases (PAKs) which are activated by autophosphorylation following binding of the GTP-bound form of the small G-protein Cdc42 (for reviews see [  1,   2,   3,   4 and   5]).	bind
18902	2	6064	7	NULL	NULL	NULL	NULL	Pak2	GP		is a type of					p21-activated protein kinases	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_515_1_84_s_3	11943200	-PAK (Pak2) is a ubiquitous member of the family of p21-activated protein kinases (PAKs) which are activated by autophosphorylation following binding of the GTP-bound form of the small G-protein Cdc42 (for reviews see [  1,   2,   3,   4 and   5]).	bind
18903	3	6064	7	NULL	NULL	NULL	NULL	PAKs	GP		is activated by					autophosphorylation	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_515_1_84_s_3	11943200	-PAK (Pak2) is a ubiquitous member of the family of p21-activated protein kinases (PAKs) which are activated by autophosphorylation following binding of the GTP-bound form of the small G-protein Cdc42 (for reviews see [  1,   2,   3,   4 and   5]).	bind
18904	4	6064	7	NULL	NULL	NULL	NULL	statement 3	Process		occurs upon					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_515_1_84_s_3	11943200	-PAK (Pak2) is a ubiquitous member of the family of p21-activated protein kinases (PAKs) which are activated by autophosphorylation following binding of the GTP-bound form of the small G-protein Cdc42 (for reviews see [  1,   2,   3,   4 and   5]).	bind
18905	5	6064	7	NULL	NULL	NULL	NULL	PAKs	GP		is					p21-activated protein kinases 	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_515_1_84_s_3	11943200	-PAK (Pak2) is a ubiquitous member of the family of p21-activated protein kinases (PAKs) which are activated by autophosphorylation following binding of the GTP-bound form of the small G-protein Cdc42 (for reviews see [  1,   2,   3,   4 and   5]).	bind
44845	6	6064	7	NULL	NULL	NULL	NULL	Cdc42	GP		is a type of					small G protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_515_1_84_s_3	11943200	-PAK (Pak2) is a ubiquitous member of the family of p21-activated protein kinases (PAKs) which are activated by autophosphorylation following binding of the GTP-bound form of the small G-protein Cdc42 (for reviews see [  1,   2,   3,   4 and   5]).	bind
15864	2	6065	5	NULL	NULL	0	NULL	PYR	NULL		bind	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_febslett_565_1_65_s_83	15135054	-PYR binding to ATP-bound DnaK monitored by tryptophan fluorescence.	bind
45615	1	6065	5	NULL	NULL	0	NULL	ATP	NULL		bind	NULL				DnaK	NULL				NULL		0	NULL	NULL	NULL	gw70_febslett_565_1_65_s_83	15135054	-PYR binding to ATP-bound DnaK monitored by tryptophan fluorescence.	bind
18907	2	6065	7	NULL	NULL	NULL	NULL	PYR	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_febslett_565_1_65_s_83	15135054	-PYR binding to ATP-bound DnaK monitored by tryptophan fluorescence.	bind
44933	1	6065	7	NULL	NULL	NULL	NULL	ATP	Chemical		bind					DnaK	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_febslett_565_1_65_s_83	15135054	-PYR binding to ATP-bound DnaK monitored by tryptophan fluorescence.	bind
15865	1	6067	5	NULL	NULL	0	NULL	Ser	NULL		bind	NULL				NMDA receptor	NULL		glycine site		NULL		0	NULL	NULL	NULL	gw60_neuroscience_83_2_449_s_179	9460753	-Ser can also bind and modulate the glycine site of the NMDA receptor.	bind
15866	2	6067	5	NULL	NULL	0	NULL	Ser	NULL		modulate	NULL				NMDA receptor	NULL		glycine site		NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_83_2_449_s_179	9460753	-Ser can also bind and modulate the glycine site of the NMDA receptor.	bind
18909	1	6067	7	NULL	NULL	NULL	NULL	Ser	AminoAcid		bind					NMDA receptor	GP		 glycine site		NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_83_2_449_s_179	9460753	-Ser can also bind and modulate the glycine site of the NMDA receptor.	bind
18911	2	6067	7	NULL	NULL	NULL	NULL	Ser	AminoAcid		modulate					NMDA receptor	GP		glycine site		NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_83_2_449_s_179	9460753	-Ser can also bind and modulate the glycine site of the NMDA receptor.	bind
15867	1	6068	5	NULL	NULL	0	NULL	Serine	NULL		does not enhance	NULL					NULL	binding of	glutamate		NULL		NULL	NULL	NULL	NULL	gw60_brainres_771_2_292_s_228	9401750	-Serine, an agonist at the glycine binding site of NMDA receptors, failed to enhance the binding of  -glutamate (data not shown).	bind
15868	2	6068	5	NULL	NULL	0	NULL	Serine	NULL		is a type of	NULL				agonist	NULL				NULL		NULL	NULL	NULL	NULL	gw60_brainres_771_2_292_s_228	9401750	-Serine, an agonist at the glycine binding site of NMDA receptors, failed to enhance the binding of  -glutamate (data not shown).	bind
25661	3	6068	5	NULL	NULL	0	NULL	Serine	NULL		is present at	NULL				NMDA receptors	NULL		glycine binding site		NULL		0	NULL	NULL	NULL	gw60_brainres_771_2_292_s_228	9401750	-Serine, an agonist at the glycine binding site of NMDA receptors, failed to enhance the binding of  -glutamate (data not shown).	bind
18914	1	6068	7	NULL	NULL	NULL	NULL	Serine	AminoAcid		is a type of					agonist	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_brainres_771_2_292_s_228	9401750	-Serine, an agonist at the glycine binding site of NMDA receptors, failed to enhance the binding of  -glutamate (data not shown).	bind
18915	3	6068	7	NULL	NULL	NULL	NULL	Serine	AminoAcid		failed to enhance					glutamate	AminoAcid	binding of			NULL		NULL	NULL	NULL	NULL	gw60_brainres_771_2_292_s_228	9401750	-Serine, an agonist at the glycine binding site of NMDA receptors, failed to enhance the binding of  -glutamate (data not shown).	bind
25660	2	6068	7	NULL	NULL	NULL	NULL	Serine	AminoAcid		is present at					NMDA receptors	GP		glycine binding site		NULL		NULL	NULL	NULL	NULL	gw60_brainres_771_2_292_s_228	9401750	-Serine, an agonist at the glycine binding site of NMDA receptors, failed to enhance the binding of  -glutamate (data not shown).	bind
15869	1	6069	5	NULL	NULL	0	NULL	Synuclein	NULL		bind	NULL				tau	NULL				NULL		0	NULL	NULL	NULL	gw70_neurobioldis_16_1_92_s_267	15207266	-Synuclein  binds to  tau and stimulates the protein kinase A-catalyzed tau phosphorylation of serine residues  263 and 356.	bind
15870	2	6069	5	NULL	NULL	0	NULL	protein kinase A	NULL		catalyze	NULL				tau	NULL	phosphorylation of	serine 263		NULL		0	NULL	NULL	NULL	gw70_neurobioldis_16_1_92_s_267	15207266	-Synuclein  binds to  tau and stimulates the protein kinase A-catalyzed tau phosphorylation of serine residues  263 and 356.	bind
15871	3	6069	5	NULL	NULL	0	NULL	protein kinase A	NULL		catalyze	NULL				tau	NULL	phosphorylation of	serine 356		NULL		0	NULL	NULL	NULL	gw70_neurobioldis_16_1_92_s_267	15207266	-Synuclein  binds to  tau and stimulates the protein kinase A-catalyzed tau phosphorylation of serine residues  263 and 356.	bind
15872	4	6069	5	NULL	NULL	0	NULL	statement 1	NULL		stimulate	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_neurobioldis_16_1_92_s_267	15207266	-Synuclein  binds to  tau and stimulates the protein kinase A-catalyzed tau phosphorylation of serine residues  263 and 356.	bind
15873	5	6069	5	NULL	NULL	0	NULL	statement 1	NULL		stimulate	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_neurobioldis_16_1_92_s_267	15207266	-Synuclein  binds to  tau and stimulates the protein kinase A-catalyzed tau phosphorylation of serine residues  263 and 356.	bind
18916	1	6069	7	NULL	NULL	NULL	NULL	Synuclein	GP		binds to					tau 	GP				NULL		NULL	NULL	NULL	NULL	gw70_neurobioldis_16_1_92_s_267	15207266	-Synuclein  binds to  tau and stimulates the protein kinase A-catalyzed tau phosphorylation of serine residues  263 and 356.	bind
18917	2	6069	7	NULL	NULL	NULL	NULL	statement 1	Process		stimulates					tau 	GP	phosphorylation  of	serine residues 263		NULL		NULL	NULL	NULL	NULL	gw70_neurobioldis_16_1_92_s_267	15207266	-Synuclein  binds to  tau and stimulates the protein kinase A-catalyzed tau phosphorylation of serine residues  263 and 356.	bind
18918	3	6069	7	NULL	NULL	NULL	NULL	statement 1	Process		stimulates					tau	GP	phosphorylation of	serine residues 356		NULL		NULL	NULL	NULL	NULL	gw70_neurobioldis_16_1_92_s_267	15207266	-Synuclein  binds to  tau and stimulates the protein kinase A-catalyzed tau phosphorylation of serine residues  263 and 356.	bind
18919	4	6069	7	NULL	NULL	NULL	NULL	protein kinase A	GP		catalyses					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_neurobioldis_16_1_92_s_267	15207266	-Synuclein  binds to  tau and stimulates the protein kinase A-catalyzed tau phosphorylation of serine residues  263 and 356.	bind
18920	5	6069	7	NULL	NULL	NULL	NULL	protein kinase A	GP		catalyses					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_neurobioldis_16_1_92_s_267	15207266	-Synuclein  binds to  tau and stimulates the protein kinase A-catalyzed tau phosphorylation of serine residues  263 and 356.	bind
15874	1	6070	5	NULL	NULL	0	NULL	Synuclein	NULL		bind	NULL				phospholipid vesicles	NULL	synthetic			NULL		0	NULL	NULL	NULL	gw60_progneurophychbiolphych_27_1_103_s_42	12551731	-Synuclein binding to synthetic phospholipid vesicles is accompanied by a strong increase in  -helicity, an observation consistent with a role in vesicle function at synaptic terminals  ( Davidson et al., 1998).	bind
15875	2	6070	5	10	NULL	0	NULL	statement 1	NULL		is accompanied by	NULL				helicity	NULL	strong increase of			NULL		NULL	NULL	NULL	NULL	gw60_progneurophychbiolphych_27_1_103_s_42	12551731	-Synuclein binding to synthetic phospholipid vesicles is accompanied by a strong increase in  -helicity, an observation consistent with a role in vesicle function at synaptic terminals  ( Davidson et al., 1998).	bind
18921	1	6070	7	NULL	NULL	NULL	NULL	Synuclein	GP		bind					phospholipid vesicles	CellComponent	synthetic			NULL		NULL	NULL	NULL	NULL	gw60_progneurophychbiolphych_27_1_103_s_42	12551731	-Synuclein binding to synthetic phospholipid vesicles is accompanied by a strong increase in  -helicity, an observation consistent with a role in vesicle function at synaptic terminals  ( Davidson et al., 1998).	bind
18922	2	6070	7	NULL	NULL	NULL	NULL	statement 1	Process		is accompanied by					helicity	Process	strong increase in			NULL		NULL	NULL	NULL	NULL	gw60_progneurophychbiolphych_27_1_103_s_42	12551731	-Synuclein binding to synthetic phospholipid vesicles is accompanied by a strong increase in  -helicity, an observation consistent with a role in vesicle function at synaptic terminals  ( Davidson et al., 1998).	bind
15876	1	6071	5	NULL	NULL	0	NULL	Synuclein	NULL		bind	NULL				tubulin	NULL				NULL		0	NULL	NULL	NULL	gw60_brainresmolbrainres_95_1_138_s_125	11687285	-Synuclein binds a tubulin affinity column	bind
18923	1	6071	7	NULL	NULL	NULL	NULL	Synuclein	GP		binds 					tubulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_95_1_138_s_125	11687285	-Synuclein binds a tubulin affinity column	bind
15877	1	6073	5	NULL	NULL	0	NULL	Synuclein	NULL		bind	NULL				synphilin-1	NULL				NULL		0	NULL	NULL	NULL	gw60_brainres_926_1_42_s_199	11814405	-Synuclein can bind to synphilin-1 and stimulate the formation of aggregates [  9 and   41].	bind
15878	2	6073	5	10	NULL	0	NULL	statement 1			stimulate					aggregates		formation of			NULL		NULL	NULL	NULL	NULL	gw60_brainres_926_1_42_s_199	11814405	-Synuclein can bind to synphilin-1 and stimulate the formation of aggregates [  9 and   41].	bind
18924	1	6073	7	NULL	NULL	NULL	NULL	Synuclein	GP		bind					synphilin-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainres_926_1_42_s_199	11814405	-Synuclein can bind to synphilin-1 and stimulate the formation of aggregates [  9 and   41].	bind
18925	2	6073	7	NULL	NULL	NULL	NULL	statement 1	Process		stimulate					aggregates	Process	formation of			NULL		NULL	NULL	NULL	NULL	gw60_brainres_926_1_42_s_199	11814405	-Synuclein can bind to synphilin-1 and stimulate the formation of aggregates [  9 and   41].	bind
15879	1	6074	5	10	NULL	0	NULL	Thrombin	NULL	purified;; radiolabeled	bind	NULL				GP Ib fragments	NULL	immobilized;; recombinant			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_16_9571_s_56	7721887	-Thrombin Binding to Immobilized Recombinant GP  Ib   Fragments -Thrombin, a generous gift of Dr. John W.  Fenton II (Wadsworth Center for Laboratory and Research and Departments  of Physiology and Biochemistry, Albany Medical College, Union  University, Albany, NY), was purified and characterized as described  previously  ( 25) ; it was radiolabeled with  I using  the IODO-GEN technique  ( 20) , as reported in detail in a  previous publication  ( 4) .	bind
18926	1	6074	7	NULL	NULL	NULL	NULL	Thrombin	GP	purified;; radiolabeled	binds to					GP Ib Fragments	AminoAcid	Immobilized;; Recombinant			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_16_9571_s_56	7721887	-Thrombin Binding to Immobilized Recombinant GP  Ib   Fragments -Thrombin, a generous gift of Dr. John W.  Fenton II (Wadsworth Center for Laboratory and Research and Departments  of Physiology and Biochemistry, Albany Medical College, Union  University, Albany, NY), was purified and characterized as described  previously  ( 25) ; it was radiolabeled with  I using  the IODO-GEN technique  ( 20) , as reported in detail in a  previous publication  ( 4) .	bind
15880	1	6075	5	NULL	NULL	0	NULL	tubulin	NULL		bind	NULL		N-site		GTP	NULL				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_13_0_83_s_47	9442869	-tubulin also binds GTP, but this  GTP is bound in a non-exchangeable manner (at the N-site) and is not hydrolyzed during  polymerization ( Spiegelman et al 1977).	bind
15881	2	6075	5	NULL	NULL	0	NULL	GTP	NULL		is not hydrolyzed	NULL				polymerization	NULL	during			NULL		0	NULL	NULL	NULL	gw70_annurevcelldevbiol_13_0_83_s_47	9442869	-tubulin also binds GTP, but this  GTP is bound in a non-exchangeable manner (at the N-site) and is not hydrolyzed during  polymerization ( Spiegelman et al 1977).	bind
25664	3	6075	5	NULL	NULL	0	NULL	statement 1	NULL		occurs in	NULL				non-exchangeable manner	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevcelldevbiol_13_0_83_s_47	9442869	-tubulin also binds GTP, but this  GTP is bound in a non-exchangeable manner (at the N-site) and is not hydrolyzed during  polymerization ( Spiegelman et al 1977).	bind
18927	1	6075	7	NULL	NULL	NULL	NULL	tubulin 	GP		binds			N-site		GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_13_0_83_s_47	9442869	-tubulin also binds GTP, but this  GTP is bound in a non-exchangeable manner (at the N-site) and is not hydrolyzed during  polymerization ( Spiegelman et al 1977).	bind
18928	2	6075	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs in a					non-exchangeable manner	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_13_0_83_s_47	9442869	-tubulin also binds GTP, but this  GTP is bound in a non-exchangeable manner (at the N-site) and is not hydrolyzed during  polymerization ( Spiegelman et al 1977).	bind
18929	3	6075	7	NULL	NULL	NULL	NULL	statement 1	Process		is not hydrolysed					polymerization 	Process	during			NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_13_0_83_s_47	9442869	-tubulin also binds GTP, but this  GTP is bound in a non-exchangeable manner (at the N-site) and is not hydrolyzed during  polymerization ( Spiegelman et al 1977).	bind
15882	1	6080	5	NULL	NULL	0	NULL	HSCO	NULL		is	NULL				hepatoma subtracted clone 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_44_46204_s_242	15302862	0610025L15Rik is 92% homologous to human HSCO (hepatoma subtracted clone 1), which binds to NF-kappaB, inhibits apoptosis and is overexpressed in hepatocellular carcinomas ( ).	bind
15883	2	6080	5	NULL	NULL	0	NULL	HSCO	NULL	human	bind	NULL				NF-kappaB	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_44_46204_s_242	15302862	0610025L15Rik is 92% homologous to human HSCO (hepatoma subtracted clone 1), which binds to NF-kappaB, inhibits apoptosis and is overexpressed in hepatocellular carcinomas ( ).	bind
15884	3	6080	5	NULL	NULL	0	NULL	HSCO	NULL	human	inhibit	NULL				apoptosis	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_44_46204_s_242	15302862	0610025L15Rik is 92% homologous to human HSCO (hepatoma subtracted clone 1), which binds to NF-kappaB, inhibits apoptosis and is overexpressed in hepatocellular carcinomas ( ).	bind
15885	4	6080	5	NULL	NULL	0	NULL	HSCO	NULL	human	is overexpressed in	NULL				hepatocellular carcinomas	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_44_46204_s_242	15302862	0610025L15Rik is 92% homologous to human HSCO (hepatoma subtracted clone 1), which binds to NF-kappaB, inhibits apoptosis and is overexpressed in hepatocellular carcinomas ( ).	bind
25662	5	6080	5	NULL	NULL	0	NULL	HSCO	NULL	human	is homologous to	NULL	mostly			0610025L15Rik	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_44_46204_s_242	15302862	0610025L15Rik is 92% homologous to human HSCO (hepatoma subtracted clone 1), which binds to NF-kappaB, inhibits apoptosis and is overexpressed in hepatocellular carcinomas ( ).	bind
18930	1	6080	7	NULL	NULL	NULL	NULL	HSCO	Cell	human	binds to					NF-kappaB	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_46204_s_242	15302862	0610025L15Rik is 92% homologous to human HSCO (hepatoma subtracted clone 1), which binds to NF-kappaB, inhibits apoptosis and is overexpressed in hepatocellular carcinomas ( ).	bind
18931	2	6080	7	NULL	NULL	NULL	NULL	statement 1	Process		inhibits					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_46204_s_242	15302862	0610025L15Rik is 92% homologous to human HSCO (hepatoma subtracted clone 1), which binds to NF-kappaB, inhibits apoptosis and is overexpressed in hepatocellular carcinomas ( ).	bind
18932	3	6080	7	NULL	NULL	NULL	NULL	HSCO	Cell	human	is overexpressed in					hepatocellular carcinomas	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_46204_s_242	15302862	0610025L15Rik is 92% homologous to human HSCO (hepatoma subtracted clone 1), which binds to NF-kappaB, inhibits apoptosis and is overexpressed in hepatocellular carcinomas ( ).	bind
18933	4	6080	7	NULL	NULL	NULL	NULL	0610025L15Rik	Cell		 homologous to		mostly			HSCO	Cell	human			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_46204_s_242	15302862	0610025L15Rik is 92% homologous to human HSCO (hepatoma subtracted clone 1), which binds to NF-kappaB, inhibits apoptosis and is overexpressed in hepatocellular carcinomas ( ).	bind
18934	5	6080	7	NULL	NULL	NULL	NULL	HSCO	Cell		is					hepatoma subtracted clone 1	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_46204_s_242	15302862	0610025L15Rik is 92% homologous to human HSCO (hepatoma subtracted clone 1), which binds to NF-kappaB, inhibits apoptosis and is overexpressed in hepatocellular carcinomas ( ).	bind
15888	1	6103	5	NULL	NULL	0	NULL	serine protease factor VII/VIIa	NULL	plasma	bind	NULL				factor IX	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_7_1804_s_15	10397701	1  2 3  It forms a complex with the plasma serine protease factor VII/VIIa, which binds and activates factors IX and X.	bind
15890	2	6103	5	NULL	NULL	0	NULL	serine protease factor VII/VIIa	NULL	plasma	activate	NULL				factor IX	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_7_1804_s_15	10397701	1  2 3  It forms a complex with the plasma serine protease factor VII/VIIa, which binds and activates factors IX and X.	bind
15891	3	6103	5	NULL	NULL	0	NULL	serine protease factor VII/VIIa	NULL	plasma	bind	NULL				factor X	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_7_1804_s_15	10397701	1  2 3  It forms a complex with the plasma serine protease factor VII/VIIa, which binds and activates factors IX and X.	bind
15892	4	6103	5	NULL	NULL	0	NULL	serine protease factor VII/VIIa	NULL	plasma	activate	NULL				factor X	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_7_1804_s_15	10397701	1  2 3  It forms a complex with the plasma serine protease factor VII/VIIa, which binds and activates factors IX and X.	bind
19054	1	6103	7	NULL	NULL	NULL	NULL	serine protease factor VII/VIIa	GP	plasma	binds					factors IX	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_7_1804_s_15	10397701	1  2 3  It forms a complex with the plasma serine protease factor VII/VIIa, which binds and activates factors IX and X.	bind
19055	2	6103	7	NULL	NULL	NULL	NULL	serine protease factor VII/VIIa	GP	plasma	binds					factor X	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_7_1804_s_15	10397701	1  2 3  It forms a complex with the plasma serine protease factor VII/VIIa, which binds and activates factors IX and X.	bind
19056	3	6103	7	NULL	NULL	NULL	NULL	serine protease factor VII/VIIa	GP	plasma	activates					factor IX	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_7_1804_s_15	10397701	1  2 3  It forms a complex with the plasma serine protease factor VII/VIIa, which binds and activates factors IX and X.	bind
19057	4	6103	7	NULL	NULL	NULL	NULL	serine protease factor VII/VIIa	GP	plasma	activates					factor X	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_7_1804_s_15	10397701	1  2 3  It forms a complex with the plasma serine protease factor VII/VIIa, which binds and activates factors IX and X.	bind
15894	1	6104	5	NULL	NULL	0	NULL	vWF	NULL	vessel-wall bound	bind	NULL				platelet GPIb-alpha	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_3_324_s_119	10645930	1  2 5 6  Under high-shear flow conditions, the vessel-wall bound vWF binds to the platelet GPIb-alpha in the early phases of hemostasis (platelet adhesion), a process independent of ADP and induced by ristocetin.	bind
15895	2	6104	5	NULL	NULL	0	NULL	hemostasis	NULL		is independent of	NULL				ADP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_3_324_s_119	10645930	1  2 5 6  Under high-shear flow conditions, the vessel-wall bound vWF binds to the platelet GPIb-alpha in the early phases of hemostasis (platelet adhesion), a process independent of ADP and induced by ristocetin.	bind
15896	3	6104	5	NULL	NULL	0	NULL	ristocetin	NULL		induce	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_101_3_324_s_119	10645930	1  2 5 6  Under high-shear flow conditions, the vessel-wall bound vWF binds to the platelet GPIb-alpha in the early phases of hemostasis (platelet adhesion), a process independent of ADP and induced by ristocetin.	bind
25663	4	6104	5	10	NULL	0	NULL	statement 1	NULL		occurs in	NULL				hemostasis 	NULL	early phases of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_3_324_s_119	10645930	1  2 5 6  Under high-shear flow conditions, the vessel-wall bound vWF binds to the platelet GPIb-alpha in the early phases of hemostasis (platelet adhesion), a process independent of ADP and induced by ristocetin.	bind
18935	1	6104	7	NULL	NULL	NULL	NULL	vWF 	GP	 vessel-wall bound 	binds to					platelet GPIb-alpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_3_324_s_119	10645930	1  2 5 6  Under high-shear flow conditions, the vessel-wall bound vWF binds to the platelet GPIb-alpha in the early phases of hemostasis (platelet adhesion), a process independent of ADP and induced by ristocetin.	bind
18936	2	6104	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs in the					hemostasis	Process	early phase of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_3_324_s_119	10645930	1  2 5 6  Under high-shear flow conditions, the vessel-wall bound vWF binds to the platelet GPIb-alpha in the early phases of hemostasis (platelet adhesion), a process independent of ADP and induced by ristocetin.	bind
18937	3	6104	7	NULL	NULL	NULL	NULL	hemostasis	Process		is independent of					ADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_3_324_s_119	10645930	1  2 5 6  Under high-shear flow conditions, the vessel-wall bound vWF binds to the platelet GPIb-alpha in the early phases of hemostasis (platelet adhesion), a process independent of ADP and induced by ristocetin.	bind
18938	4	6104	7	NULL	NULL	NULL	NULL	ristocetin	Chemical		induce					hemostasis	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_3_324_s_119	10645930	1  2 5 6  Under high-shear flow conditions, the vessel-wall bound vWF binds to the platelet GPIb-alpha in the early phases of hemostasis (platelet adhesion), a process independent of ADP and induced by ristocetin.	bind
15897	1	6106	5	NULL	NULL	0	NULL	heparin polysaccharide chains	NULL		bind	NULL	high affinity			antithrombin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_16_9043_s_14	7721817	1  and 2) The accelerating activity results from a sequence-specific  pentasaccharide region, present in about one-third of heparin  polysaccharide chains  ( 3,  4,  5) , which binds  antithrombin with high affinity and induces an activating  conformational change in the inhibitor  ( 6,  7,  8,  9,  10,  11) .	bind
15899	2	6106	5	10	NULL	0	NULL	statement 1			induce					inhibitor		activating;; conformational change in			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_16_9043_s_14	7721817	1  and 2) The accelerating activity results from a sequence-specific  pentasaccharide region, present in about one-third of heparin  polysaccharide chains  ( 3,  4,  5) , which binds  antithrombin with high affinity and induces an activating  conformational change in the inhibitor  ( 6,  7,  8,  9,  10,  11) .	bind
18939	1	6106	7	NULL	NULL	NULL	NULL	heparin	GP		binds		high affinity	polysaccharide chains		antithrombin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_16_9043_s_14	7721817	1  and 2) The accelerating activity results from a sequence-specific  pentasaccharide region, present in about one-third of heparin  polysaccharide chains  ( 3,  4,  5) , which binds  antithrombin with high affinity and induces an activating  conformational change in the inhibitor  ( 6,  7,  8,  9,  10,  11) .	bind
18940	2	6106	7	NULL	NULL	NULL	NULL	statement 1	Process		induce					inhibitor	Chemical	activating;; conformational change in			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_16_9043_s_14	7721817	1  and 2) The accelerating activity results from a sequence-specific  pentasaccharide region, present in about one-third of heparin  polysaccharide chains  ( 3,  4,  5) , which binds  antithrombin with high affinity and induces an activating  conformational change in the inhibitor  ( 6,  7,  8,  9,  10,  11) .	bind
15900	1	6107	5	NULL	NULL	0	NULL	LDL	NULL		bind	NULL				proteoglycans	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_5_1340_s_21	10323788	1  Binding of LDL to proteoglycans traps LDL in the arterial intima, which provides the opportunity for oxidation of LDL lipids.	bind
15902	2	6107	5	10	NULL	0	NULL	statement 1	NULL		traps	NULL				LDL	NULL				NULL	arterial intima	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_5_1340_s_21	10323788	1  Binding of LDL to proteoglycans traps LDL in the arterial intima, which provides the opportunity for oxidation of LDL lipids.	bind
15903	3	6107	5	10	NULL	0	NULL	statement 2	NULL		plays a role in	NULL				LDL lipids	NULL	oxidation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_5_1340_s_21	10323788	1  Binding of LDL to proteoglycans traps LDL in the arterial intima, which provides the opportunity for oxidation of LDL lipids.	bind
18949	1	6107	7	NULL	NULL	NULL	NULL	LDL	Chemical		bind					proteoglycans	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_5_1340_s_21	10323788	1  Binding of LDL to proteoglycans traps LDL in the arterial intima, which provides the opportunity for oxidation of LDL lipids.	bind
18950	2	6107	7	NULL	NULL	NULL	NULL	statement 1	Process		traps					LDL	Chemical				NULL	in the arterial intima	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_5_1340_s_21	10323788	1  Binding of LDL to proteoglycans traps LDL in the arterial intima, which provides the opportunity for oxidation of LDL lipids.	bind
18951	3	6107	7	NULL	NULL	NULL	NULL	statement 2	Process		plays a role in					LDL lipids	Chemical	oxidation of 			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_5_1340_s_21	10323788	1  Binding of LDL to proteoglycans traps LDL in the arterial intima, which provides the opportunity for oxidation of LDL lipids.	bind
15905	1	6108	5	NULL	NULL	0	NULL	VLDL	NULL	from patients homozygous for apo E2/2	bind	NULL				VLDL receptor	NULL	human			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_8_1142_s_28	11222479	1  Furthermore, VLDL from patients homozygous for apo E2/2 and apo E3/3 binds the human VLDL receptor identically.	bind
15906	2	6108	5	NULL	NULL	0	NULL	VLDL	NULL	from patients homozygous for apo E3/3	bind	NULL				VLDL receptor	NULL	human			NULL		0	NULL	NULL	NULL	gw60_circulation_103_8_1142_s_28	11222479	1  Furthermore, VLDL from patients homozygous for apo E2/2 and apo E3/3 binds the human VLDL receptor identically.	bind
15907	3	6108	5	NULL	NULL	0	NULL	statement 1	NULL		identical to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_8_1142_s_28	11222479	1  Furthermore, VLDL from patients homozygous for apo E2/2 and apo E3/3 binds the human VLDL receptor identically.	bind
18952	1	6108	7	NULL	NULL	NULL	NULL	apo E2/2	Chemical		binds					 VLDL receptor	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_8_1142_s_28	11222479	1  Furthermore, VLDL from patients homozygous for apo E2/2 and apo E3/3 binds the human VLDL receptor identically.	bind
18953	2	6108	7	NULL	NULL	NULL	NULL	apo E3/3	Chemical		binds					VLDL receptor	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_8_1142_s_28	11222479	1  Furthermore, VLDL from patients homozygous for apo E2/2 and apo E3/3 binds the human VLDL receptor identically.	bind
18954	3	6108	7	NULL	NULL	NULL	NULL	statement 1	Process		is identical to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_8_1142_s_28	11222479	1  Furthermore, VLDL from patients homozygous for apo E2/2 and apo E3/3 binds the human VLDL receptor identically.	bind
15910	1	6109	5	NULL	NULL	0	NULL	PU.1	NULL		is necessary for	NULL		Ets DNA binding domain		nuclear localization 	NULL				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_j-biol-chem_280_11_15632149_s_4	15632149	1  fusions, we show that the Ets DNA binding domain of PU.1 is necessary  and sufficient for its nuclear localization.	bind
15911	2	6109	5	NULL	NULL	0	NULL	PU.1	NULL		is sufficient for	NULL		Ets DNA binding domain		nuclear localization	NULL				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_j-biol-chem_280_11_15632149_s_4	15632149	1  fusions, we show that the Ets DNA binding domain of PU.1 is necessary  and sufficient for its nuclear localization.	bind
18955	1	6109	7	NULL	NULL	NULL	NULL	PU.1	GP		is necessary for			Ets DNA binding domain		nuclear localization	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-biol-chem_280_11_15632149_s_4	15632149	1  fusions, we show that the Ets DNA binding domain of PU.1 is necessary  and sufficient for its nuclear localization.	bind
25665	2	6109	7	NULL	NULL	NULL	NULL	PU.1	GP		is sufficient for			Ets DNA binding domain		nuclear localization	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-biol-chem_280_11_15632149_s_4	15632149	1  fusions, we show that the Ets DNA binding domain of PU.1 is necessary  and sufficient for its nuclear localization.	bind
15912	1	6110	5	NULL	NULL	0	NULL	Heparin s 	NULL		bind	NULL				antithrombin	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2162_s_17	10978264	1  Heparin s binding to antithrombin produces a conformational change in antithrombin that considerably accelerates the ability of the latter to inactivate coagulation enzymes.	bind
15913	2	6110	5	NULL	NULL	0	NULL	statement 1	NULL		produce	NULL				antithrombin	NULL	conformation change in			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2162_s_17	10978264	1  Heparin s binding to antithrombin produces a conformational change in antithrombin that considerably accelerates the ability of the latter to inactivate coagulation enzymes.	bind
15914	3	6110	5	NULL	NULL	0	NULL	antithrombin	NULL		inactivate	NULL				coagulation enzymes	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2162_s_17	10978264	1  Heparin s binding to antithrombin produces a conformational change in antithrombin that considerably accelerates the ability of the latter to inactivate coagulation enzymes.	bind
15915	4	6110	5	NULL	NULL	0	NULL	statement 2	NULL		accelerates	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2162_s_17	10978264	1  Heparin s binding to antithrombin produces a conformational change in antithrombin that considerably accelerates the ability of the latter to inactivate coagulation enzymes.	bind
18956	1	6110	7	NULL	NULL	NULL	NULL	Heparin s	GP		bind					antithrombin	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2162_s_17	10978264	1  Heparin s binding to antithrombin produces a conformational change in antithrombin that considerably accelerates the ability of the latter to inactivate coagulation enzymes.	bind
18957	2	6110	7	NULL	NULL	NULL	NULL	statement 1	Process		produces					antithrombin	GP	conformational change in			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2162_s_17	10978264	1  Heparin s binding to antithrombin produces a conformational change in antithrombin that considerably accelerates the ability of the latter to inactivate coagulation enzymes.	bind
18958	3	6110	7	NULL	NULL	NULL	NULL	antithrombin	GP		inactivate					coagulation enzymes	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2162_s_17	10978264	1  Heparin s binding to antithrombin produces a conformational change in antithrombin that considerably accelerates the ability of the latter to inactivate coagulation enzymes.	bind
18959	4	6110	7	NULL	NULL	NULL	NULL	statement 2	Process		accelerates					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2162_s_17	10978264	1  Heparin s binding to antithrombin produces a conformational change in antithrombin that considerably accelerates the ability of the latter to inactivate coagulation enzymes.	bind
15916	1	6111	5	10	NULL	0	NULL	G-protein-coupled receptor	NULL	human	is similar to	NULL				GPR14	NULL	rat			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_10_1378_s_17	11245639	1  In 1999, Ames et al 4  cloned a human G-protein-coupled receptor, similar to the rat GPR14, which selectively bound human UII (hUII).	bind
15917	2	6111	5	10	NULL	0	NULL	G-protein-coupled receptor	NULL	human	bind	NULL	selectively			hUII	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_10_1378_s_17	11245639	1  In 1999, Ames et al 4  cloned a human G-protein-coupled receptor, similar to the rat GPR14, which selectively bound human UII (hUII).	bind
15918	3	6111	5	NULL	NULL	0	NULL	hUII	NULL		is	NULL				human UII	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_10_1378_s_17	11245639	1  In 1999, Ames et al 4  cloned a human G-protein-coupled receptor, similar to the rat GPR14, which selectively bound human UII (hUII).	bind
18960	1	6111	7	NULL	NULL	NULL	NULL	G-protein-coupled receptor	GP	human	bind		selectively			hUII	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_10_1378_s_17	11245639	1  In 1999, Ames et al 4  cloned a human G-protein-coupled receptor, similar to the rat GPR14, which selectively bound human UII (hUII).	bind
18962	2	6111	7	NULL	NULL	NULL	NULL	GPR14	GP	rat	is similar to					G-protein-coupled receptor	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_10_1378_s_17	11245639	1  In 1999, Ames et al 4  cloned a human G-protein-coupled receptor, similar to the rat GPR14, which selectively bound human UII (hUII).	bind
18963	3	6111	7	NULL	NULL	NULL	NULL	hUII	GP		is					human UII	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_10_1378_s_17	11245639	1  In 1999, Ames et al 4  cloned a human G-protein-coupled receptor, similar to the rat GPR14, which selectively bound human UII (hUII).	bind
15919	1	6112	5	NULL	NULL	0	NULL	thrombin	NULL		bind	NULL				thrombomodulin	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_2_547_s_12	9708814	1  It is activated by thrombin bound to thrombomodulin, an endothelial cell surface protein.	bind
54150	2	6112	5	10	NULL	0	NULL	thrombomodulin			is a type of					endothelial cell surface protein					NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_2_547_s_12	9708814	1  It is activated by thrombin bound to thrombomodulin, an endothelial cell surface protein.	bind
18964	1	6112	7	NULL	NULL	NULL	NULL	thrombin	GP		bind					thrombomodulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_2_547_s_12	9708814	1  It is activated by thrombin bound to thrombomodulin, an endothelial cell surface protein.	bind
18965	2	6112	7	NULL	NULL	NULL	NULL	thrombomodulin	GP		is a type of					endothelial cell surface protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_2_547_s_12	9708814	1  It is activated by thrombin bound to thrombomodulin, an endothelial cell surface protein.	bind
15920	1	6113	5	NULL	NULL	0	NULL	LDL receptors	NULL	reduced activity of	leads to	NULL	may			LDL - apo B	NULL	high levels of 			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_4_517_s_18	8624773	1  Several mechanisms may lead to high levels of LDL - apo B; these include reduced activity of LDL receptors, 3  defective apo B that prevents normal binding of LDL to LDL receptors, 4 5 6 7  and possibly overproduction of apo B - containing lipoproteins by the liver.	bind
15921	2	6113	5	NULL	NULL	0	NULL	LDL	NULL		bind	NULL				LDL receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_4_517_s_18	8624773	1  Several mechanisms may lead to high levels of LDL - apo B; these include reduced activity of LDL receptors, 3  defective apo B that prevents normal binding of LDL to LDL receptors, 4 5 6 7  and possibly overproduction of apo B - containing lipoproteins by the liver.	bind
15922	3	6113	5	NULL	NULL	0	NULL	apo B	NULL	defective	prevent	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_4_517_s_18	8624773	1  Several mechanisms may lead to high levels of LDL - apo B; these include reduced activity of LDL receptors, 3  defective apo B that prevents normal binding of LDL to LDL receptors, 4 5 6 7  and possibly overproduction of apo B - containing lipoproteins by the liver.	bind
15923	4	6113	5	NULL	NULL	0	NULL	statement 3	NULL		leads to	NULL	may			LDL - apo B	NULL	high levels of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_4_517_s_18	8624773	1  Several mechanisms may lead to high levels of LDL - apo B; these include reduced activity of LDL receptors, 3  defective apo B that prevents normal binding of LDL to LDL receptors, 4 5 6 7  and possibly overproduction of apo B - containing lipoproteins by the liver.	bind
15925	5	6113	5	NULL	NULL	0	NULL	liver	NULL		overproduce	NULL				lipoproteins	NULL	apo B - containing			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_4_517_s_18	8624773	1  Several mechanisms may lead to high levels of LDL - apo B; these include reduced activity of LDL receptors, 3  defective apo B that prevents normal binding of LDL to LDL receptors, 4 5 6 7  and possibly overproduction of apo B - containing lipoproteins by the liver.	bind
15926	6	6113	5	NULL	NULL	0	NULL	statement 5	NULL		leads to	NULL	may			LDL - apo B	NULL	high levels of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_4_517_s_18	8624773	1  Several mechanisms may lead to high levels of LDL - apo B; these include reduced activity of LDL receptors, 3  defective apo B that prevents normal binding of LDL to LDL receptors, 4 5 6 7  and possibly overproduction of apo B - containing lipoproteins by the liver.	bind
18966	1	6113	7	NULL	NULL	NULL	NULL	LDL - apo B	GP	high levels of	is due to					LDL receptor	GP	reduced activity of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_4_517_s_18	8624773	1  Several mechanisms may lead to high levels of LDL - apo B; these include reduced activity of LDL receptors, 3  defective apo B that prevents normal binding of LDL to LDL receptors, 4 5 6 7  and possibly overproduction of apo B - containing lipoproteins by the liver.	bind
18967	2	6113	7	NULL	NULL	NULL	NULL	LDL	GP		bind					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_4_517_s_18	8624773	1  Several mechanisms may lead to high levels of LDL - apo B; these include reduced activity of LDL receptors, 3  defective apo B that prevents normal binding of LDL to LDL receptors, 4 5 6 7  and possibly overproduction of apo B - containing lipoproteins by the liver.	bind
18969	3	6113	7	NULL	NULL	NULL	NULL	apoB	Chemical	defective	prevents					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_4_517_s_18	8624773	1  Several mechanisms may lead to high levels of LDL - apo B; these include reduced activity of LDL receptors, 3  defective apo B that prevents normal binding of LDL to LDL receptors, 4 5 6 7  and possibly overproduction of apo B - containing lipoproteins by the liver.	bind
23899	5	6113	7	NULL	NULL	NULL	NULL	liver	OrganismPart		overproduce					lipoproteins	GP	apo B - containing			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_4_517_s_18	8624773	1  Several mechanisms may lead to high levels of LDL - apo B; these include reduced activity of LDL receptors, 3  defective apo B that prevents normal binding of LDL to LDL receptors, 4 5 6 7  and possibly overproduction of apo B - containing lipoproteins by the liver.	bind
23900	4	6113	7	NULL	NULL	NULL	NULL	statement 3	Process		leads to		may			LDL - apo B	GP	high levels of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_4_517_s_18	8624773	1  Several mechanisms may lead to high levels of LDL - apo B; these include reduced activity of LDL receptors, 3  defective apo B that prevents normal binding of LDL to LDL receptors, 4 5 6 7  and possibly overproduction of apo B - containing lipoproteins by the liver.	bind
23901	6	6113	7	NULL	NULL	NULL	NULL	statement 5	Process		leads to		may			LDL-apoB	GP	high levels of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_4_517_s_18	8624773	1  Several mechanisms may lead to high levels of LDL - apo B; these include reduced activity of LDL receptors, 3  defective apo B that prevents normal binding of LDL to LDL receptors, 4 5 6 7  and possibly overproduction of apo B - containing lipoproteins by the liver.	bind
15927	1	6115	5	NULL	NULL	0	NULL	SR-A	NULL		is	NULL				macrophage scavenger receptor A	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_5_825_s_14	11348881	1  The human macrophage scavenger receptor A (SR-A) binds and internalizes modified LDL, which ultimately results in the accumulation of cholesterol esters in macrophages.	bind
15928	2	6115	5	10	NULL	0	NULL	SR-A	NULL	human;; macrophage	bind	NULL				LDL	NULL	modified			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_5_825_s_14	11348881	1  The human macrophage scavenger receptor A (SR-A) binds and internalizes modified LDL, which ultimately results in the accumulation of cholesterol esters in macrophages.	bind
15929	3	6115	5	NULL	NULL	0	NULL	SR-A	NULL		internalize	NULL				LDL	NULL	modified			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_5_825_s_14	11348881	1  The human macrophage scavenger receptor A (SR-A) binds and internalizes modified LDL, which ultimately results in the accumulation of cholesterol esters in macrophages.	bind
15932	4	6115	5	NULL	NULL	0	NULL	statement 3	NULL		results in	NULL				cholesterol esters	NULL	accumulation of 			NULL	in macrophages	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_5_825_s_14	11348881	1  The human macrophage scavenger receptor A (SR-A) binds and internalizes modified LDL, which ultimately results in the accumulation of cholesterol esters in macrophages.	bind
18972	1	6115	7	NULL	NULL	NULL	NULL	SR-A	GP	human;;macrophage	binds					LDL	GP	modified			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_5_825_s_14	11348881	1  The human macrophage scavenger receptor A (SR-A) binds and internalizes modified LDL, which ultimately results in the accumulation of cholesterol esters in macrophages.	bind
18973	2	6115	7	NULL	NULL	NULL	NULL	statement 1	Process		internalizes					LDL	GP	modified			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_5_825_s_14	11348881	1  The human macrophage scavenger receptor A (SR-A) binds and internalizes modified LDL, which ultimately results in the accumulation of cholesterol esters in macrophages.	bind
18974	3	6115	7	NULL	NULL	NULL	NULL	statement 2	Process		results in					cholesterol esters	Chemical	accumulation of			NULL	in macrophages	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_5_825_s_14	11348881	1  The human macrophage scavenger receptor A (SR-A) binds and internalizes modified LDL, which ultimately results in the accumulation of cholesterol esters in macrophages.	bind
18975	4	6115	7	NULL	NULL	NULL	NULL	SR-A	GP		is					scavenger receptor A	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_5_825_s_14	11348881	1  The human macrophage scavenger receptor A (SR-A) binds and internalizes modified LDL, which ultimately results in the accumulation of cholesterol esters in macrophages.	bind
16011	1	6116	5	NULL	NULL	0	NULL	beta2-integrin	NULL		bind	NULL				fibrinogen	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_13_1772_s_26	11282909	1  Their cooperative cellular interactions are mediated by adhesion molecules, ie, P-selectin or beta2- and beta3-integrins binding to fibrinogen, and contribute to thrombus formation and fibrin deposition.	bind
16012	2	6116	5	NULL	NULL	0	NULL	beta3-integrin	NULL		bind	NULL				fibrinogen	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_13_1772_s_26	11282909	1  Their cooperative cellular interactions are mediated by adhesion molecules, ie, P-selectin or beta2- and beta3-integrins binding to fibrinogen, and contribute to thrombus formation and fibrin deposition.	bind
24518	3	6116	5	NULL	NULL	0	NULL	P-selectin	NULL		bind	NULL				fibrinogen	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_13_1772_s_26	11282909	1  Their cooperative cellular interactions are mediated by adhesion molecules, ie, P-selectin or beta2- and beta3-integrins binding to fibrinogen, and contribute to thrombus formation and fibrin deposition.	bind
24520	4	6116	5	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_13_1772_s_26	11282909	1  Their cooperative cellular interactions are mediated by adhesion molecules, ie, P-selectin or beta2- and beta3-integrins binding to fibrinogen, and contribute to thrombus formation and fibrin deposition.	bind
24521	5	6116	5	NULL	NULL	0	NULL	statement 2	NULL		is an alternative to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_13_1772_s_26	11282909	1  Their cooperative cellular interactions are mediated by adhesion molecules, ie, P-selectin or beta2- and beta3-integrins binding to fibrinogen, and contribute to thrombus formation and fibrin deposition.	bind
24527	6	6116	5	NULL	NULL	0	NULL	statement 1	NULL		contribute to	NULL				thrombus	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_circulation_103_13_1772_s_26	11282909	1  Their cooperative cellular interactions are mediated by adhesion molecules, ie, P-selectin or beta2- and beta3-integrins binding to fibrinogen, and contribute to thrombus formation and fibrin deposition.	bind
24528	7	6116	5	NULL	NULL	0	NULL	statement 2	NULL		contribute to	NULL				thrombus	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_circulation_103_13_1772_s_26	11282909	1  Their cooperative cellular interactions are mediated by adhesion molecules, ie, P-selectin or beta2- and beta3-integrins binding to fibrinogen, and contribute to thrombus formation and fibrin deposition.	bind
24529	8	6116	5	NULL	NULL	0	NULL	statement 3	NULL		contribute to	NULL				thrombus	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_circulation_103_13_1772_s_26	11282909	1  Their cooperative cellular interactions are mediated by adhesion molecules, ie, P-selectin or beta2- and beta3-integrins binding to fibrinogen, and contribute to thrombus formation and fibrin deposition.	bind
24530	9	6116	5	NULL	NULL	0	NULL	statement 1	NULL		contribute to	NULL				fibrin	NULL	deposition of			NULL		0	NULL	NULL	NULL	gw60_circulation_103_13_1772_s_26	11282909	1  Their cooperative cellular interactions are mediated by adhesion molecules, ie, P-selectin or beta2- and beta3-integrins binding to fibrinogen, and contribute to thrombus formation and fibrin deposition.	bind
24531	10	6116	5	NULL	NULL	0	NULL	statement 2	NULL		contribute to	NULL				fibrin	NULL	deposition of			NULL		0	NULL	NULL	NULL	gw60_circulation_103_13_1772_s_26	11282909	1  Their cooperative cellular interactions are mediated by adhesion molecules, ie, P-selectin or beta2- and beta3-integrins binding to fibrinogen, and contribute to thrombus formation and fibrin deposition.	bind
24532	11	6116	5	NULL	NULL	0	NULL	statement 3	NULL		contribute to	NULL				fibrin	NULL	deposition of			NULL		0	NULL	NULL	NULL	gw60_circulation_103_13_1772_s_26	11282909	1  Their cooperative cellular interactions are mediated by adhesion molecules, ie, P-selectin or beta2- and beta3-integrins binding to fibrinogen, and contribute to thrombus formation and fibrin deposition.	bind
18976	1	6116	7	NULL	NULL	NULL	NULL	P-selectin	GP		bind					fibrinogen	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_13_1772_s_26	11282909	1  Their cooperative cellular interactions are mediated by adhesion molecules, ie, P-selectin or beta2- and beta3-integrins binding to fibrinogen, and contribute to thrombus formation and fibrin deposition.	bind
18977	2	6116	7	NULL	NULL	NULL	NULL	beta2- integrins	GP		bind					fibrinogen	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_13_1772_s_26	11282909	1  Their cooperative cellular interactions are mediated by adhesion molecules, ie, P-selectin or beta2- and beta3-integrins binding to fibrinogen, and contribute to thrombus formation and fibrin deposition.	bind
18978	3	6116	7	NULL	NULL	NULL	NULL	beta3-integrins	GP		bind					fibrinogen	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_13_1772_s_26	11282909	1  Their cooperative cellular interactions are mediated by adhesion molecules, ie, P-selectin or beta2- and beta3-integrins binding to fibrinogen, and contribute to thrombus formation and fibrin deposition.	bind
18979	4	6116	7	NULL	NULL	NULL	NULL	statement 1	Process		contribute to					thrombus	GP	formation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_13_1772_s_26	11282909	1  Their cooperative cellular interactions are mediated by adhesion molecules, ie, P-selectin or beta2- and beta3-integrins binding to fibrinogen, and contribute to thrombus formation and fibrin deposition.	bind
18980	5	6116	7	NULL	NULL	NULL	NULL	statement 2	Process		contribute to					thrombus	GP	formation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_13_1772_s_26	11282909	1  Their cooperative cellular interactions are mediated by adhesion molecules, ie, P-selectin or beta2- and beta3-integrins binding to fibrinogen, and contribute to thrombus formation and fibrin deposition.	bind
18981	6	6116	7	NULL	NULL	NULL	NULL	statement 3	Process		contribute to					thrombus	GP	formation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_13_1772_s_26	11282909	1  Their cooperative cellular interactions are mediated by adhesion molecules, ie, P-selectin or beta2- and beta3-integrins binding to fibrinogen, and contribute to thrombus formation and fibrin deposition.	bind
18982	7	6116	7	NULL	NULL	NULL	NULL	statement 1	Process		leads to					fibrin	GP	deposition of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_13_1772_s_26	11282909	1  Their cooperative cellular interactions are mediated by adhesion molecules, ie, P-selectin or beta2- and beta3-integrins binding to fibrinogen, and contribute to thrombus formation and fibrin deposition.	bind
18983	8	6116	7	NULL	NULL	NULL	NULL	statement 2	Process		leads to					fibrin	GP	deposition of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_13_1772_s_26	11282909	1  Their cooperative cellular interactions are mediated by adhesion molecules, ie, P-selectin or beta2- and beta3-integrins binding to fibrinogen, and contribute to thrombus formation and fibrin deposition.	bind
18984	9	6116	7	NULL	NULL	NULL	NULL	statement 3	Process		leads to					fibrin	GP	deposition of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_13_1772_s_26	11282909	1  Their cooperative cellular interactions are mediated by adhesion molecules, ie, P-selectin or beta2- and beta3-integrins binding to fibrinogen, and contribute to thrombus formation and fibrin deposition.	bind
18985	10	6116	7	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_13_1772_s_26	11282909	1  Their cooperative cellular interactions are mediated by adhesion molecules, ie, P-selectin or beta2- and beta3-integrins binding to fibrinogen, and contribute to thrombus formation and fibrin deposition.	bind
18986	11	6116	7	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_13_1772_s_26	11282909	1  Their cooperative cellular interactions are mediated by adhesion molecules, ie, P-selectin or beta2- and beta3-integrins binding to fibrinogen, and contribute to thrombus formation and fibrin deposition.	bind
16013	1	6117	5	NULL	NULL	0	NULL	(IgG1,kappa) antibody	NULL		bind	NULL				CD11a	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_48_30463_s_34	9374538	1 ( 17) and TS1/22 ( 15) (IgG1,kappa) antibodies that bind to CD11a; 44 ( 18), an (IgG1,kappa) antibody that binds to CD11b; and 3.9 ( 19) an (IgG1,kappa) antibody that binds to CD11c.	bind
16014	2	6117	5	NULL	NULL	0	NULL	(IgG1,kappa) antibody	NULL		bind	NULL				CD11b	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_48_30463_s_34	9374538	1 ( 17) and TS1/22 ( 15) (IgG1,kappa) antibodies that bind to CD11a; 44 ( 18), an (IgG1,kappa) antibody that binds to CD11b; and 3.9 ( 19) an (IgG1,kappa) antibody that binds to CD11c.	bind
16015	3	6117	5	NULL	NULL	0	NULL	(IgG1,kappa) antibody	NULL		bind	NULL				CD11c	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_48_30463_s_34	9374538	1 ( 17) and TS1/22 ( 15) (IgG1,kappa) antibodies that bind to CD11a; 44 ( 18), an (IgG1,kappa) antibody that binds to CD11b; and 3.9 ( 19) an (IgG1,kappa) antibody that binds to CD11c.	bind
18989	1	6117	7	NULL	NULL	NULL	NULL	IgG1,kappa antibody	GP		bind					CD11a	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_48_30463_s_34	9374538	1 ( 17) and TS1/22 ( 15) (IgG1,kappa) antibodies that bind to CD11a; 44 ( 18), an (IgG1,kappa) antibody that binds to CD11b; and 3.9 ( 19) an (IgG1,kappa) antibody that binds to CD11c.	bind
18990	2	6117	7	NULL	NULL	NULL	NULL	IgG1,kappa antibody	GP		bind					CD11b	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_48_30463_s_34	9374538	1 ( 17) and TS1/22 ( 15) (IgG1,kappa) antibodies that bind to CD11a; 44 ( 18), an (IgG1,kappa) antibody that binds to CD11b; and 3.9 ( 19) an (IgG1,kappa) antibody that binds to CD11c.	bind
18992	3	6117	7	NULL	NULL	NULL	NULL	IgG1,kappa antibody	GP		bind					CD11c	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_48_30463_s_34	9374538	1 ( 17) and TS1/22 ( 15) (IgG1,kappa) antibodies that bind to CD11a; 44 ( 18), an (IgG1,kappa) antibody that binds to CD11b; and 3.9 ( 19) an (IgG1,kappa) antibody that binds to CD11c.	bind
16016	1	6118	5	NULL	NULL	0	NULL	tissue factor	NULL		bind	NULL				factor VII	NULL	activated			NULL		0	NULL	NULL	NULL	gw60_circulation_105_15_1756_s_24	11956113	1 -  4 This cascade is initiated by binding of tissue factor to activated factor VII, and this complex activates factor X.	bind
16017	2	6118	5	NULL	NULL	0	NULL	statement 1	NULL		activates	NULL				factor X	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_15_1756_s_24	11956113	1 -  4 This cascade is initiated by binding of tissue factor to activated factor VII, and this complex activates factor X.	bind
18993	1	6118	7	NULL	NULL	NULL	NULL	tissue factor	GP		bind					factor VII	GP	activated			NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_15_1756_s_24	11956113	1 -  4 This cascade is initiated by binding of tissue factor to activated factor VII, and this complex activates factor X.	bind
18994	2	6118	7	NULL	NULL	NULL	NULL	statement 1	Process		activates					factor X	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_15_1756_s_24	11956113	1 -  4 This cascade is initiated by binding of tissue factor to activated factor VII, and this complex activates factor X.	bind
16019	1	6119	5	NULL	NULL	0	NULL	beta1-adrenergic receptor	NULL		bind	NULL				catecholamines	NULL	circulating			NULL		0	NULL	NULL	NULL	gw60_circulationres_89_11_997_s_10	11717156	1 -  5 The beta1- and beta2-adrenergic receptors (betaARs), which bind circulating catecholamines, activate adenylyl cyclase by coupling through the stimulatory G-protein, Galphas.	bind
16020	2	6119	5	NULL	NULL	0	NULL	beta2-adrenergic receptor	NULL		bind	NULL				catecholamines	NULL	circulating			NULL		0	NULL	NULL	NULL	gw60_circulationres_89_11_997_s_10	11717156	1 -  5 The beta1- and beta2-adrenergic receptors (betaARs), which bind circulating catecholamines, activate adenylyl cyclase by coupling through the stimulatory G-protein, Galphas.	bind
16021	3	6119	5	NULL	NULL	0	NULL	beta1-adrenergic receptor	NULL		activate	NULL				adenylyl cyclase	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_89_11_997_s_10	11717156	1 -  5 The beta1- and beta2-adrenergic receptors (betaARs), which bind circulating catecholamines, activate adenylyl cyclase by coupling through the stimulatory G-protein, Galphas.	bind
16022	4	6119	5	NULL	NULL	0	NULL	beta2-adrenergic receptor	NULL		activate	NULL				adenylyl cyclase	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_89_11_997_s_10	11717156	1 -  5 The beta1- and beta2-adrenergic receptors (betaARs), which bind circulating catecholamines, activate adenylyl cyclase by coupling through the stimulatory G-protein, Galphas.	bind
16023	5	6119	5	NULL	NULL	0	NULL	beta1-adrenergic receptor	NULL		couple through	NULL				Galphas	NULL	stimulatory G-protein			NULL		0	NULL	NULL	NULL	gw60_circulationres_89_11_997_s_10	11717156	1 -  5 The beta1- and beta2-adrenergic receptors (betaARs), which bind circulating catecholamines, activate adenylyl cyclase by coupling through the stimulatory G-protein, Galphas.	bind
16024	6	6119	5	NULL	NULL	0	NULL	beta2-adrenergic receptor	NULL		couple through	NULL				Galphas	NULL	stimulatory G-protein			NULL		0	NULL	NULL	NULL	gw60_circulationres_89_11_997_s_10	11717156	1 -  5 The beta1- and beta2-adrenergic receptors (betaARs), which bind circulating catecholamines, activate adenylyl cyclase by coupling through the stimulatory G-protein, Galphas.	bind
16025	7	6119	5	NULL	NULL	0	NULL	statement 5	NULL		leads to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_89_11_997_s_10	11717156	1 -  5 The beta1- and beta2-adrenergic receptors (betaARs), which bind circulating catecholamines, activate adenylyl cyclase by coupling through the stimulatory G-protein, Galphas.	bind
16026	8	6119	5	NULL	NULL	0	NULL	statement 6	NULL		leads to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_89_11_997_s_10	11717156	1 -  5 The beta1- and beta2-adrenergic receptors (betaARs), which bind circulating catecholamines, activate adenylyl cyclase by coupling through the stimulatory G-protein, Galphas.	bind
24533	9	6119	5	NULL	NULL	0	NULL	betaARs	NULL		is	NULL				beta-adrenergic receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_89_11_997_s_10	11717156	1 -  5 The beta1- and beta2-adrenergic receptors (betaARs), which bind circulating catecholamines, activate adenylyl cyclase by coupling through the stimulatory G-protein, Galphas.	bind
18995	1	6119	7	NULL	NULL	NULL	NULL	beta1adrenergic receptor	GP		bind					catecholamines	Chemical	circulating			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_89_11_997_s_10	11717156	1 -  5 The beta1- and beta2-adrenergic receptors (betaARs), which bind circulating catecholamines, activate adenylyl cyclase by coupling through the stimulatory G-protein, Galphas.	bind
18996	2	6119	7	NULL	NULL	NULL	NULL	beta2-adrenergic receptor	GP		bind					catecholamines	Chemical	circulating			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_89_11_997_s_10	11717156	1 -  5 The beta1- and beta2-adrenergic receptors (betaARs), which bind circulating catecholamines, activate adenylyl cyclase by coupling through the stimulatory G-protein, Galphas.	bind
18997	3	6119	7	NULL	NULL	NULL	NULL	statement 1	Process		activate					adenylyl cyclase	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_89_11_997_s_10	11717156	1 -  5 The beta1- and beta2-adrenergic receptors (betaARs), which bind circulating catecholamines, activate adenylyl cyclase by coupling through the stimulatory G-protein, Galphas.	bind
18998	4	6119	7	NULL	NULL	NULL	NULL	statement 2	Process		activate					adenylyl cyclase	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_89_11_997_s_10	11717156	1 -  5 The beta1- and beta2-adrenergic receptors (betaARs), which bind circulating catecholamines, activate adenylyl cyclase by coupling through the stimulatory G-protein, Galphas.	bind
18999	5	6119	7	NULL	NULL	NULL	NULL	statement 3	Process		occurs through					Galphas	GP	stimulatory G-protein			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_89_11_997_s_10	11717156	1 -  5 The beta1- and beta2-adrenergic receptors (betaARs), which bind circulating catecholamines, activate adenylyl cyclase by coupling through the stimulatory G-protein, Galphas.	bind
19001	6	6119	7	NULL	NULL	NULL	NULL	statement 4	Process		occurs through					Galphas	GP	stimulatory G-protein			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_89_11_997_s_10	11717156	1 -  5 The beta1- and beta2-adrenergic receptors (betaARs), which bind circulating catecholamines, activate adenylyl cyclase by coupling through the stimulatory G-protein, Galphas.	bind
19002	7	6119	7	NULL	NULL	NULL	NULL	betaARs	GP		is					beta-adrenergic receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_89_11_997_s_10	11717156	1 -  5 The beta1- and beta2-adrenergic receptors (betaARs), which bind circulating catecholamines, activate adenylyl cyclase by coupling through the stimulatory G-protein, Galphas.	bind
23902	8	6119	7	NULL	NULL	NULL	NULL	statement 5	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_89_11_997_s_10	11717156	1 -  5 The beta1- and beta2-adrenergic receptors (betaARs), which bind circulating catecholamines, activate adenylyl cyclase by coupling through the stimulatory G-protein, Galphas.	bind
23903	9	6119	7	NULL	NULL	NULL	NULL	statement 6	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_89_11_997_s_10	11717156	1 -  5 The beta1- and beta2-adrenergic receptors (betaARs), which bind circulating catecholamines, activate adenylyl cyclase by coupling through the stimulatory G-protein, Galphas.	bind
16027	1	6121	5	10	NULL	0	NULL	cAMP			bind					PKA			regulatory subunit 		NULL	eukaryotes	NULL	NULL	NULL	NULL	gw60_circulationres_88_3_319_s_12	11179200	1 2  In eukaryotes, cAMP binds the regulatory subunit of cAMP-dependent protein kinases (PKAs).	bind
16028	2	6121	5	NULL	NULL	0	NULL	PKAs	NULL		is	NULL				cAMP-dependent protein kinases	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_3_319_s_12	11179200	1 2  In eukaryotes, cAMP binds the regulatory subunit of cAMP-dependent protein kinases (PKAs).	bind
19006	1	6121	7	NULL	NULL	NULL	NULL	cAMP	Chemical		binds					PKA	GP		regulatory subunit 		NULL	in eukaryotes	NULL	NULL	NULL	NULL	gw60_circulationres_88_3_319_s_12	11179200	1 2  In eukaryotes, cAMP binds the regulatory subunit of cAMP-dependent protein kinases (PKAs).	bind
19007	2	6121	7	NULL	NULL	NULL	NULL	PKA	GP		is					cAMP-dependent protein kinases	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_3_319_s_12	11179200	1 2  In eukaryotes, cAMP binds the regulatory subunit of cAMP-dependent protein kinases (PKAs).	bind
16029	1	6122	5	NULL	NULL	0	NULL	heme	NULL		bind	NULL				NAD(P)H oxidases	NULL		p22phox subunit		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_4_365_s_3	10700437	1 2  In this issue of  Circulation Research, Cahilly and colleagues 3  provide data supporting an association between a histidine72 to tyrosine mutation at the potential site for heme binding of the p22phox subunit of NAD(P)H oxidases and increased severity and progression of CAD in patients from the Lipoprotein and Coronary Atherosclerosis Study (LCAS).	bind
16030	2	6122	5	NULL	NULL	0	NULL		NULL		is associated to	NULL		histidine72		statement 1	NULL	mutation at potential site for	tyrosine		NULL		0	NULL	NULL	NULL	gw60_circulationres_86_4_365_s_3	10700437	1 2  In this issue of  Circulation Research, Cahilly and colleagues 3  provide data supporting an association between a histidine72 to tyrosine mutation at the potential site for heme binding of the p22phox subunit of NAD(P)H oxidases and increased severity and progression of CAD in patients from the Lipoprotein and Coronary Atherosclerosis Study (LCAS).	bind
19053	1	6122	7	NULL	NULL	NULL	NULL	NAD(P)H oxidases	GP		bind			p22phox subunit 		heme 	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_4_365_s_3	10700437	1 2  In this issue of  Circulation Research, Cahilly and colleagues 3  provide data supporting an association between a histidine72 to tyrosine mutation at the potential site for heme binding of the p22phox subunit of NAD(P)H oxidases and increased severity and progression of CAD in patients from the Lipoprotein and Coronary Atherosclerosis Study (LCAS).	bind
23904	2	6122	7	NULL	NULL	NULL	NULL				is associated to			histidine72		statement 1	Process	mutation at the potential site for	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_4_365_s_3	10700437	1 2  In this issue of  Circulation Research, Cahilly and colleagues 3  provide data supporting an association between a histidine72 to tyrosine mutation at the potential site for heme binding of the p22phox subunit of NAD(P)H oxidases and increased severity and progression of CAD in patients from the Lipoprotein and Coronary Atherosclerosis Study (LCAS).	bind
16031	1	6123	5	NULL	NULL	0	NULL	GC-A	NULL		is	NULL				guanylate cyclase-A	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_930_s_25	11397699	1 2  These peptides elicit their biological effects via the elevation of intracellular cGMP by activating 2 biologically active natriuretic peptide receptors, namely, membrane-bound guanylate cyclase-A (GC-A) and guanylate cyclase-B (GC-B).	bind
16032	2	6123	5	NULL	NULL	0	NULL	GC-B	NULL		is	NULL				guanylate cyclase-B	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_930_s_25	11397699	1 2  These peptides elicit their biological effects via the elevation of intracellular cGMP by activating 2 biologically active natriuretic peptide receptors, namely, membrane-bound guanylate cyclase-A (GC-A) and guanylate cyclase-B (GC-B).	bind
16033	3	6123	5	10	NULL	0	NULL	GC-A	NULL		elevate	NULL				cGMP	NULL	intracellular			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_930_s_25	11397699	1 2  These peptides elicit their biological effects via the elevation of intracellular cGMP by activating 2 biologically active natriuretic peptide receptors, namely, membrane-bound guanylate cyclase-A (GC-A) and guanylate cyclase-B (GC-B).	bind
16035	4	6123	5	10	NULL	0	NULL	GC-B	NULL		elevate	NULL				cGMP	NULL	intracellular			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_930_s_25	11397699	1 2  These peptides elicit their biological effects via the elevation of intracellular cGMP by activating 2 biologically active natriuretic peptide receptors, namely, membrane-bound guanylate cyclase-A (GC-A) and guanylate cyclase-B (GC-B).	bind
45131	5	6123	5	10	NULL	0	NULL	GC-A	NULL		is a type of	NULL				biologically active natriuretic peptide receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_930_s_25	11397699	1 2  These peptides elicit their biological effects via the elevation of intracellular cGMP by activating 2 biologically active natriuretic peptide receptors, namely, membrane-bound guanylate cyclase-A (GC-A) and guanylate cyclase-B (GC-B).	bind
45132	6	6123	5	10	NULL	0	NULL	GC-B	NULL		is a type of	NULL				biologically active natriuretic peptide receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_930_s_25	11397699	1 2  These peptides elicit their biological effects via the elevation of intracellular cGMP by activating 2 biologically active natriuretic peptide receptors, namely, membrane-bound guanylate cyclase-A (GC-A) and guanylate cyclase-B (GC-B).	bind
19063	1	6123	7	NULL	NULL	NULL	NULL	GC-A	GP		elevates					cGMP	Chemical	intracellular			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_930_s_25	11397699	1 2  These peptides elicit their biological effects via the elevation of intracellular cGMP by activating 2 biologically active natriuretic peptide receptors, namely, membrane-bound guanylate cyclase-A (GC-A) and guanylate cyclase-B (GC-B).	bind
19064	2	6123	7	NULL	NULL	NULL	NULL	GC-B	GP		elevates					cGMP	Chemical	intracellular			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_930_s_25	11397699	1 2  These peptides elicit their biological effects via the elevation of intracellular cGMP by activating 2 biologically active natriuretic peptide receptors, namely, membrane-bound guanylate cyclase-A (GC-A) and guanylate cyclase-B (GC-B).	bind
19065	3	6123	7	NULL	NULL	NULL	NULL	GC-A	GP		is					guanylate cyclase-A	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_930_s_25	11397699	1 2  These peptides elicit their biological effects via the elevation of intracellular cGMP by activating 2 biologically active natriuretic peptide receptors, namely, membrane-bound guanylate cyclase-A (GC-A) and guanylate cyclase-B (GC-B).	bind
19066	4	6123	7	NULL	NULL	NULL	NULL	GC-B	GP		is					guanylate cyclase-B	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_930_s_25	11397699	1 2  These peptides elicit their biological effects via the elevation of intracellular cGMP by activating 2 biologically active natriuretic peptide receptors, namely, membrane-bound guanylate cyclase-A (GC-A) and guanylate cyclase-B (GC-B).	bind
45134	5	6123	7	NULL	NULL	NULL	NULL	GC-A	GP		is a type of					biologically active natriuretic peptide receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_930_s_25	11397699	1 2  These peptides elicit their biological effects via the elevation of intracellular cGMP by activating 2 biologically active natriuretic peptide receptors, namely, membrane-bound guanylate cyclase-A (GC-A) and guanylate cyclase-B (GC-B).	bind
45135	6	6123	7	NULL	NULL	NULL	NULL	GC-B	GP		is a type of					biologically active natriuretic peptide receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_930_s_25	11397699	1 2  These peptides elicit their biological effects via the elevation of intracellular cGMP by activating 2 biologically active natriuretic peptide receptors, namely, membrane-bound guanylate cyclase-A (GC-A) and guanylate cyclase-B (GC-B).	bind
16037	1	6124	5	NULL	NULL	0	NULL	fibrinogen	NULL		bind	NULL				GPIIb/IIa	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_149_s_20	11145947	1 2  This adhesion step is followed by aggregation predominantly mediated by the binding of fibrinogen and vWF to GPIIb/IIa in the presence of ADP. 1 2 3 4  In addition, direct platelet aggregation in the bulk phase under conditions of abnormally elevated fluid shear stresses, analogous to those occurring in atherosclerotic or constricted arterial vessels, 5  may be important.	bind
16039	2	6124	5	NULL	NULL	0	NULL	statement 1	NULL		in the presence of	NULL				ADP	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_149_s_20	11145947	1 2  This adhesion step is followed by aggregation predominantly mediated by the binding of fibrinogen and vWF to GPIIb/IIa in the presence of ADP. 1 2 3 4  In addition, direct platelet aggregation in the bulk phase under conditions of abnormally elevated fluid shear stresses, analogous to those occurring in atherosclerotic or constricted arterial vessels, 5  may be important.	bind
16040	3	6124	5	NULL	NULL	0	NULL	vWF	NULL		bind	NULL				GPIIb/IIa	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_149_s_20	11145947	1 2  This adhesion step is followed by aggregation predominantly mediated by the binding of fibrinogen and vWF to GPIIb/IIa in the presence of ADP. 1 2 3 4  In addition, direct platelet aggregation in the bulk phase under conditions of abnormally elevated fluid shear stresses, analogous to those occurring in atherosclerotic or constricted arterial vessels, 5  may be important.	bind
16041	4	6124	5	NULL	NULL	0	NULL	statement 3	NULL		in the presence of	NULL				ADP	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_149_s_20	11145947	1 2  This adhesion step is followed by aggregation predominantly mediated by the binding of fibrinogen and vWF to GPIIb/IIa in the presence of ADP. 1 2 3 4  In addition, direct platelet aggregation in the bulk phase under conditions of abnormally elevated fluid shear stresses, analogous to those occurring in atherosclerotic or constricted arterial vessels, 5  may be important.	bind
16043	5	6124	5	NULL	NULL	0	NULL	statement 2	NULL		mediate	NULL				aggregation	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_149_s_20	11145947	1 2  This adhesion step is followed by aggregation predominantly mediated by the binding of fibrinogen and vWF to GPIIb/IIa in the presence of ADP. 1 2 3 4  In addition, direct platelet aggregation in the bulk phase under conditions of abnormally elevated fluid shear stresses, analogous to those occurring in atherosclerotic or constricted arterial vessels, 5  may be important.	bind
16044	6	6124	5	NULL	NULL	0	NULL	statement 4	NULL		mediate	NULL				aggregation	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_149_s_20	11145947	1 2  This adhesion step is followed by aggregation predominantly mediated by the binding of fibrinogen and vWF to GPIIb/IIa in the presence of ADP. 1 2 3 4  In addition, direct platelet aggregation in the bulk phase under conditions of abnormally elevated fluid shear stresses, analogous to those occurring in atherosclerotic or constricted arterial vessels, 5  may be important.	bind
16046	7	6124	5	NULL	NULL	0	NULL	adhesion	NULL		is followed by	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_149_s_20	11145947	1 2  This adhesion step is followed by aggregation predominantly mediated by the binding of fibrinogen and vWF to GPIIb/IIa in the presence of ADP. 1 2 3 4  In addition, direct platelet aggregation in the bulk phase under conditions of abnormally elevated fluid shear stresses, analogous to those occurring in atherosclerotic or constricted arterial vessels, 5  may be important.	bind
16047	8	6124	5	NULL	NULL	0	NULL	adhesion	NULL		is followed by	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_149_s_20	11145947	1 2  This adhesion step is followed by aggregation predominantly mediated by the binding of fibrinogen and vWF to GPIIb/IIa in the presence of ADP. 1 2 3 4  In addition, direct platelet aggregation in the bulk phase under conditions of abnormally elevated fluid shear stresses, analogous to those occurring in atherosclerotic or constricted arterial vessels, 5  may be important.	bind
19069	1	6124	7	NULL	NULL	NULL	NULL	fibrinogen	GP		bind					GPIIb/IIa	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_149_s_20	11145947	1 2  This adhesion step is followed by aggregation predominantly mediated by the binding of fibrinogen and vWF to GPIIb/IIa in the presence of ADP. 1 2 3 4  In addition, direct platelet aggregation in the bulk phase under conditions of abnormally elevated fluid shear stresses, analogous to those occurring in atherosclerotic or constricted arterial vessels, 5  may be important.	bind
19070	2	6124	7	NULL	NULL	NULL	NULL	vWF	GP		bind					GPIIb/IIa	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_149_s_20	11145947	1 2  This adhesion step is followed by aggregation predominantly mediated by the binding of fibrinogen and vWF to GPIIb/IIa in the presence of ADP. 1 2 3 4  In addition, direct platelet aggregation in the bulk phase under conditions of abnormally elevated fluid shear stresses, analogous to those occurring in atherosclerotic or constricted arterial vessels, 5  may be important.	bind
23905	3	6124	7	NULL	NULL	NULL	NULL	statement 1	Process		in the presence of 					ADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_149_s_20	11145947	1 2  This adhesion step is followed by aggregation predominantly mediated by the binding of fibrinogen and vWF to GPIIb/IIa in the presence of ADP. 1 2 3 4  In addition, direct platelet aggregation in the bulk phase under conditions of abnormally elevated fluid shear stresses, analogous to those occurring in atherosclerotic or constricted arterial vessels, 5  may be important.	bind
23906	4	6124	7	NULL	NULL	NULL	NULL	statement 2	Process		in the presence of 					ADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_149_s_20	11145947	1 2  This adhesion step is followed by aggregation predominantly mediated by the binding of fibrinogen and vWF to GPIIb/IIa in the presence of ADP. 1 2 3 4  In addition, direct platelet aggregation in the bulk phase under conditions of abnormally elevated fluid shear stresses, analogous to those occurring in atherosclerotic or constricted arterial vessels, 5  may be important.	bind
23907	5	6124	7	NULL	NULL	NULL	NULL	statement 3	Process		mediate					aggregation	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_149_s_20	11145947	1 2  This adhesion step is followed by aggregation predominantly mediated by the binding of fibrinogen and vWF to GPIIb/IIa in the presence of ADP. 1 2 3 4  In addition, direct platelet aggregation in the bulk phase under conditions of abnormally elevated fluid shear stresses, analogous to those occurring in atherosclerotic or constricted arterial vessels, 5  may be important.	bind
23908	6	6124	7	NULL	NULL	NULL	NULL	statement 4	Process		mediate					aggregation	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_149_s_20	11145947	1 2  This adhesion step is followed by aggregation predominantly mediated by the binding of fibrinogen and vWF to GPIIb/IIa in the presence of ADP. 1 2 3 4  In addition, direct platelet aggregation in the bulk phase under conditions of abnormally elevated fluid shear stresses, analogous to those occurring in atherosclerotic or constricted arterial vessels, 5  may be important.	bind
23909	7	6124	7	NULL	NULL	NULL	NULL	Adhesion	Process		is followed by					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_149_s_20	11145947	1 2  This adhesion step is followed by aggregation predominantly mediated by the binding of fibrinogen and vWF to GPIIb/IIa in the presence of ADP. 1 2 3 4  In addition, direct platelet aggregation in the bulk phase under conditions of abnormally elevated fluid shear stresses, analogous to those occurring in atherosclerotic or constricted arterial vessels, 5  may be important.	bind
23910	8	6124	7	NULL	NULL	NULL	NULL	Adhesion	Process		is followed by					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_149_s_20	11145947	1 2  This adhesion step is followed by aggregation predominantly mediated by the binding of fibrinogen and vWF to GPIIb/IIa in the presence of ADP. 1 2 3 4  In addition, direct platelet aggregation in the bulk phase under conditions of abnormally elevated fluid shear stresses, analogous to those occurring in atherosclerotic or constricted arterial vessels, 5  may be important.	bind
16052	1	6125	5	10	NULL	0	NULL	CD8-positive T cells	NULL	cytotoxic	bind	NULL	specifically			major histocompatibility - complex	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_94_7_1665_s_21	8840859	1 2 3  Cytotoxic CD8-positive T cells bind specifically to foreign class I major histocompatibility - complexbearing target cells and release agents, eg, granzyme B, which disrupt cell membranes and may also induce apoptosis as demonstrated in vitro.	bind
16053	2	6125	5	NULL	NULL	0	NULL	CD8-positive T cells	NULL	cytotoxic	release	NULL				granzyme B	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_94_7_1665_s_21	8840859	1 2 3  Cytotoxic CD8-positive T cells bind specifically to foreign class I major histocompatibility - complexbearing target cells and release agents, eg, granzyme B, which disrupt cell membranes and may also induce apoptosis as demonstrated in vitro.	bind
16054	3	6125	5	NULL	NULL	0	NULL	granzyme B	NULL		disrupt	NULL				cell membranes	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_94_7_1665_s_21	8840859	1 2 3  Cytotoxic CD8-positive T cells bind specifically to foreign class I major histocompatibility - complexbearing target cells and release agents, eg, granzyme B, which disrupt cell membranes and may also induce apoptosis as demonstrated in vitro.	bind
16055	4	6125	5	NULL	NULL	0	NULL	granzyme B	NULL		induce	NULL	may			apoptosis	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_circulation_94_7_1665_s_21	8840859	1 2 3  Cytotoxic CD8-positive T cells bind specifically to foreign class I major histocompatibility - complexbearing target cells and release agents, eg, granzyme B, which disrupt cell membranes and may also induce apoptosis as demonstrated in vitro.	bind
19071	1	6125	7	NULL	NULL	NULL	NULL	CD8-positive T cells	Cell	Cytotoxic	bind		specifically			 major histocompatibility - complex	GP	foreign	class I		NULL		NULL	NULL	NULL	NULL	gw60_circulation_94_7_1665_s_21	8840859	1 2 3  Cytotoxic CD8-positive T cells bind specifically to foreign class I major histocompatibility - complexbearing target cells and release agents, eg, granzyme B, which disrupt cell membranes and may also induce apoptosis as demonstrated in vitro.	bind
19072	2	6125	7	NULL	NULL	NULL	NULL	CD8-positive T cells	Cell	cytotoxic	release					granzyme B	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_94_7_1665_s_21	8840859	1 2 3  Cytotoxic CD8-positive T cells bind specifically to foreign class I major histocompatibility - complexbearing target cells and release agents, eg, granzyme B, which disrupt cell membranes and may also induce apoptosis as demonstrated in vitro.	bind
19073	3	6125	7	NULL	NULL	NULL	NULL	granzyme B	GP		disrupt					cell membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_circulation_94_7_1665_s_21	8840859	1 2 3  Cytotoxic CD8-positive T cells bind specifically to foreign class I major histocompatibility - complexbearing target cells and release agents, eg, granzyme B, which disrupt cell membranes and may also induce apoptosis as demonstrated in vitro.	bind
19074	4	6125	7	NULL	NULL	NULL	NULL	granzyme B	GP		induce		may			apoptosis	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulation_94_7_1665_s_21	8840859	1 2 3  Cytotoxic CD8-positive T cells bind specifically to foreign class I major histocompatibility - complexbearing target cells and release agents, eg, granzyme B, which disrupt cell membranes and may also induce apoptosis as demonstrated in vitro.	bind
16056	1	6126	5	10	NULL	0	NULL	NP			bind		specific			cell surface receptors		characterized;;purified;;cloned from vasculature			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_8_841_s_19	10785505	1 2 3  These effects are mediated by specific binding of NP to cell surface receptors that have been characterized, purified, and cloned from the vasculature, kidney, adrenal gland, and brain.	bind
16057	2	6126	5	10	NULL	0	NULL	NP			bind		specific			cell surface receptors		characterized;;purified;;cloned from vasculature			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_8_841_s_19	10785505	1 2 3  These effects are mediated by specific binding of NP to cell surface receptors that have been characterized, purified, and cloned from the vasculature, kidney, adrenal gland, and brain.	bind
16058	3	6126	5	10	NULL	0	NULL	NP			bind		specific			cell surface receptors		characterized;;purified;;cloned from vasculature			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_8_841_s_19	10785505	1 2 3  These effects are mediated by specific binding of NP to cell surface receptors that have been characterized, purified, and cloned from the vasculature, kidney, adrenal gland, and brain.	bind
16059	4	6126	5	10	NULL	0	NULL	NP			bind		specific			cell surface receptors		characterized;;purified;;cloned from vasculature			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_8_841_s_19	10785505	1 2 3  These effects are mediated by specific binding of NP to cell surface receptors that have been characterized, purified, and cloned from the vasculature, kidney, adrenal gland, and brain.	bind
19075	1	6126	7	NULL	NULL	NULL	NULL	 NP	GP		bind		specific			cell surface receptor	GP	characterized;;purified;;cloned from vasculature			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_8_841_s_19	10785505	1 2 3  These effects are mediated by specific binding of NP to cell surface receptors that have been characterized, purified, and cloned from the vasculature, kidney, adrenal gland, and brain.	bind
24120	2	6126	7	NULL	NULL	NULL	NULL	NP	GP		bind		specific			cell surface receptor	GP	characterized;;purified;;cloned from vasculature			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_8_841_s_19	10785505	1 2 3  These effects are mediated by specific binding of NP to cell surface receptors that have been characterized, purified, and cloned from the vasculature, kidney, adrenal gland, and brain.	bind
24121	3	6126	7	NULL	NULL	NULL	NULL	NP	GP		bind		specific			cell surface receptor	GP	characterized;;purified;;cloned from vasculature			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_8_841_s_19	10785505	1 2 3  These effects are mediated by specific binding of NP to cell surface receptors that have been characterized, purified, and cloned from the vasculature, kidney, adrenal gland, and brain.	bind
24122	4	6126	7	NULL	NULL	NULL	NULL	NP	GP		bind		specific			cell surface receptor	GP	characterized;;purified;;cloned from vasculature			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_8_841_s_19	10785505	1 2 3  These effects are mediated by specific binding of NP to cell surface receptors that have been characterized, purified, and cloned from the vasculature, kidney, adrenal gland, and brain.	bind
16060	1	6127	5	NULL	NULL	0	NULL	titin	NULL	cloned	bind	NULL				F-actin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_77_4_856_s_176	7554133	1 2 3  Using cloned titin fragments, Jin 16  recently reported binding between titin and F-actin, and this interaction may underlie the inelastic behavior of titin in the I band.	bind
24535	2	6127	5	NULL	NULL	0	NULL	statement 1	NULL		underlie	NULL	may			titin	NULL	inelastic behavior of			NULL	in I band	0	NULL	NULL	NULL	gw60_circulationres_77_4_856_s_176	7554133	1 2 3  Using cloned titin fragments, Jin 16  recently reported binding between titin and F-actin, and this interaction may underlie the inelastic behavior of titin in the I band.	bind
19076	1	6127	7	NULL	NULL	NULL	NULL	titin	GP	cloned	bind					F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_4_856_s_176	7554133	1 2 3  Using cloned titin fragments, Jin 16  recently reported binding between titin and F-actin, and this interaction may underlie the inelastic behavior of titin in the I band.	bind
19077	2	6127	7	NULL	NULL	NULL	NULL	statement 1	Process		underlie					titin	GP	inelastic behaviour of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_4_856_s_176	7554133	1 2 3  Using cloned titin fragments, Jin 16  recently reported binding between titin and F-actin, and this interaction may underlie the inelastic behavior of titin in the I band.	bind
16061	1	6128	5	10	NULL	0	NULL	fluid shear stress			causes					platelet		aggregation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_6_1399_s_18	7664419	1 2 3 4  5 6 7 8 9 10 14 15 16 17  The platelet aggregation response to fluid shear stress occurs in the absence of exogenous agonists 2  3  and requires intact vWf multimers, extracellular Ca2+, endogenous ADP contained in platelet granules, and metabolically active platelets with intact platelet membrane glycoprotein (GP) Ib and [[ GP IIb/IIa. 1 2 3 4 5 6 7 8 9 10  Arterial ]] and pathological levels of shear stress (>30 dynes/cm2) initiate platelet aggregation by inducing the binding of vWf to platelet GP Ib.	bind
16062	2	6128	5	NULL	NULL	0	NULL	statement 1	NULL		in the absence of	NULL				agonists	NULL	exogenous			NULL		0	NULL	NULL	NULL	gw60_circulation_92_6_1399_s_18	7664419	1 2 3 4  5 6 7 8 9 10 14 15 16 17  The platelet aggregation response to fluid shear stress occurs in the absence of exogenous agonists 2  3  and requires intact vWf multimers, extracellular Ca2+, endogenous ADP contained in platelet granules, and metabolically active platelets with intact platelet membrane glycoprotein (GP) Ib and [[ GP IIb/IIa. 1 2 3 4 5 6 7 8 9 10  Arterial ]] and pathological levels of shear stress (>30 dynes/cm2) initiate platelet aggregation by inducing the binding of vWf to platelet GP Ib.	bind
16063	3	6128	5	NULL	NULL	0	NULL	statement 1	NULL		requires	NULL				vWf multimers	NULL	intact			NULL		0	NULL	NULL	NULL	gw60_circulation_92_6_1399_s_18	7664419	1 2 3 4  5 6 7 8 9 10 14 15 16 17  The platelet aggregation response to fluid shear stress occurs in the absence of exogenous agonists 2  3  and requires intact vWf multimers, extracellular Ca2+, endogenous ADP contained in platelet granules, and metabolically active platelets with intact platelet membrane glycoprotein (GP) Ib and [[ GP IIb/IIa. 1 2 3 4 5 6 7 8 9 10  Arterial ]] and pathological levels of shear stress (>30 dynes/cm2) initiate platelet aggregation by inducing the binding of vWf to platelet GP Ib.	bind
16064	4	6128	5	NULL	NULL	0	NULL	statement 1	NULL		requires	NULL				Ca2+	NULL	extracellular			NULL		0	NULL	NULL	NULL	gw60_circulation_92_6_1399_s_18	7664419	1 2 3 4  5 6 7 8 9 10 14 15 16 17  The platelet aggregation response to fluid shear stress occurs in the absence of exogenous agonists 2  3  and requires intact vWf multimers, extracellular Ca2+, endogenous ADP contained in platelet granules, and metabolically active platelets with intact platelet membrane glycoprotein (GP) Ib and [[ GP IIb/IIa. 1 2 3 4 5 6 7 8 9 10  Arterial ]] and pathological levels of shear stress (>30 dynes/cm2) initiate platelet aggregation by inducing the binding of vWf to platelet GP Ib.	bind
16065	5	6128	5	10	NULL	0	NULL	statement 1	NULL		requires	NULL				ADP	NULL	endogenous			NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_6_1399_s_18	7664419	1 2 3 4  5 6 7 8 9 10 14 15 16 17  The platelet aggregation response to fluid shear stress occurs in the absence of exogenous agonists 2  3  and requires intact vWf multimers, extracellular Ca2+, endogenous ADP contained in platelet granules, and metabolically active platelets with intact platelet membrane glycoprotein (GP) Ib and [[ GP IIb/IIa. 1 2 3 4 5 6 7 8 9 10  Arterial ]] and pathological levels of shear stress (>30 dynes/cm2) initiate platelet aggregation by inducing the binding of vWf to platelet GP Ib.	bind
16067	7	6128	5	10	NULL	0	NULL	statement 1	NULL		requires	NULL				platelets	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_6_1399_s_18	7664419	1 2 3 4  5 6 7 8 9 10 14 15 16 17  The platelet aggregation response to fluid shear stress occurs in the absence of exogenous agonists 2  3  and requires intact vWf multimers, extracellular Ca2+, endogenous ADP contained in platelet granules, and metabolically active platelets with intact platelet membrane glycoprotein (GP) Ib and [[ GP IIb/IIa. 1 2 3 4 5 6 7 8 9 10  Arterial ]] and pathological levels of shear stress (>30 dynes/cm2) initiate platelet aggregation by inducing the binding of vWf to platelet GP Ib.	bind
16068	8	6128	5	10	NULL	0	NULL	shear stress		pathological levels of 	initiate					platelet		aggregation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_6_1399_s_18	7664419	1 2 3 4  5 6 7 8 9 10 14 15 16 17  The platelet aggregation response to fluid shear stress occurs in the absence of exogenous agonists 2  3  and requires intact vWf multimers, extracellular Ca2+, endogenous ADP contained in platelet granules, and metabolically active platelets with intact platelet membrane glycoprotein (GP) Ib and [[ GP IIb/IIa. 1 2 3 4 5 6 7 8 9 10  Arterial ]] and pathological levels of shear stress (>30 dynes/cm2) initiate platelet aggregation by inducing the binding of vWf to platelet GP Ib.	bind
16069	9	6128	5	NULL	NULL	0	NULL	vWf	NULL		bind	NULL				GP Ib	NULL	platelet			NULL		0	NULL	NULL	NULL	gw60_circulation_92_6_1399_s_18	7664419	1 2 3 4  5 6 7 8 9 10 14 15 16 17  The platelet aggregation response to fluid shear stress occurs in the absence of exogenous agonists 2  3  and requires intact vWf multimers, extracellular Ca2+, endogenous ADP contained in platelet granules, and metabolically active platelets with intact platelet membrane glycoprotein (GP) Ib and [[ GP IIb/IIa. 1 2 3 4 5 6 7 8 9 10  Arterial ]] and pathological levels of shear stress (>30 dynes/cm2) initiate platelet aggregation by inducing the binding of vWf to platelet GP Ib.	bind
16070	10	6128	5	NULL	NULL	0	NULL	shear stress	NULL	pathological levels of	induce	NULL				statement 9	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_6_1399_s_18	7664419	1 2 3 4  5 6 7 8 9 10 14 15 16 17  The platelet aggregation response to fluid shear stress occurs in the absence of exogenous agonists 2  3  and requires intact vWf multimers, extracellular Ca2+, endogenous ADP contained in platelet granules, and metabolically active platelets with intact platelet membrane glycoprotein (GP) Ib and [[ GP IIb/IIa. 1 2 3 4 5 6 7 8 9 10  Arterial ]] and pathological levels of shear stress (>30 dynes/cm2) initiate platelet aggregation by inducing the binding of vWf to platelet GP Ib.	bind
16071	11	6128	5	NULL	NULL	0	NULL	statement 10	NULL		leads to	NULL				statement 8	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_6_1399_s_18	7664419	1 2 3 4  5 6 7 8 9 10 14 15 16 17  The platelet aggregation response to fluid shear stress occurs in the absence of exogenous agonists 2  3  and requires intact vWf multimers, extracellular Ca2+, endogenous ADP contained in platelet granules, and metabolically active platelets with intact platelet membrane glycoprotein (GP) Ib and [[ GP IIb/IIa. 1 2 3 4 5 6 7 8 9 10  Arterial ]] and pathological levels of shear stress (>30 dynes/cm2) initiate platelet aggregation by inducing the binding of vWf to platelet GP Ib.	bind
45166	6	6128	5	10	NULL	0	NULL	GPIb	NULL		is a type of	NULL				platelet membrane glycoprotein	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_6_1399_s_18	7664419	1 2 3 4  5 6 7 8 9 10 14 15 16 17  The platelet aggregation response to fluid shear stress occurs in the absence of exogenous agonists 2  3  and requires intact vWf multimers, extracellular Ca2+, endogenous ADP contained in platelet granules, and metabolically active platelets with intact platelet membrane glycoprotein (GP) Ib and [[ GP IIb/IIa. 1 2 3 4 5 6 7 8 9 10  Arterial ]] and pathological levels of shear stress (>30 dynes/cm2) initiate platelet aggregation by inducing the binding of vWf to platelet GP Ib.	bind
19081	1	6128	7	NULL	NULL	NULL	NULL	 vWf	GP		bind					GP Ib	GP	platelet			NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_6_1399_s_18	7664419	1 2 3 4  5 6 7 8 9 10 14 15 16 17  The platelet aggregation response to fluid shear stress occurs in the absence of exogenous agonists 2  3  and requires intact vWf multimers, extracellular Ca2+, endogenous ADP contained in platelet granules, and metabolically active platelets with intact platelet membrane glycoprotein (GP) Ib and [[ GP IIb/IIa. 1 2 3 4 5 6 7 8 9 10  Arterial ]] and pathological levels of shear stress (>30 dynes/cm2) initiate platelet aggregation by inducing the binding of vWf to platelet GP Ib.	bind
19082	2	6128	7	NULL	NULL	NULL	NULL	fluid shear stress	Process		aggregates					platelets	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_6_1399_s_18	7664419	1 2 3 4  5 6 7 8 9 10 14 15 16 17  The platelet aggregation response to fluid shear stress occurs in the absence of exogenous agonists 2  3  and requires intact vWf multimers, extracellular Ca2+, endogenous ADP contained in platelet granules, and metabolically active platelets with intact platelet membrane glycoprotein (GP) Ib and [[ GP IIb/IIa. 1 2 3 4 5 6 7 8 9 10  Arterial ]] and pathological levels of shear stress (>30 dynes/cm2) initiate platelet aggregation by inducing the binding of vWf to platelet GP Ib.	bind
19083	3	6128	7	NULL	NULL	NULL	NULL	statement 2	Process		in absence of					agonists	Chemical	exogenous			NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_6_1399_s_18	7664419	1 2 3 4  5 6 7 8 9 10 14 15 16 17  The platelet aggregation response to fluid shear stress occurs in the absence of exogenous agonists 2  3  and requires intact vWf multimers, extracellular Ca2+, endogenous ADP contained in platelet granules, and metabolically active platelets with intact platelet membrane glycoprotein (GP) Ib and [[ GP IIb/IIa. 1 2 3 4 5 6 7 8 9 10  Arterial ]] and pathological levels of shear stress (>30 dynes/cm2) initiate platelet aggregation by inducing the binding of vWf to platelet GP Ib.	bind
19084	4	6128	7	NULL	NULL	NULL	NULL	statement 2	Process		requires					 Ca2+	Chemical	extracellular			NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_6_1399_s_18	7664419	1 2 3 4  5 6 7 8 9 10 14 15 16 17  The platelet aggregation response to fluid shear stress occurs in the absence of exogenous agonists 2  3  and requires intact vWf multimers, extracellular Ca2+, endogenous ADP contained in platelet granules, and metabolically active platelets with intact platelet membrane glycoprotein (GP) Ib and [[ GP IIb/IIa. 1 2 3 4 5 6 7 8 9 10  Arterial ]] and pathological levels of shear stress (>30 dynes/cm2) initiate platelet aggregation by inducing the binding of vWf to platelet GP Ib.	bind
19085	5	6128	7	NULL	NULL	NULL	NULL	statement 2	Process		requires					ADP	Chemical	endogenous			NULL	in platelet granules	NULL	NULL	NULL	NULL	gw60_circulation_92_6_1399_s_18	7664419	1 2 3 4  5 6 7 8 9 10 14 15 16 17  The platelet aggregation response to fluid shear stress occurs in the absence of exogenous agonists 2  3  and requires intact vWf multimers, extracellular Ca2+, endogenous ADP contained in platelet granules, and metabolically active platelets with intact platelet membrane glycoprotein (GP) Ib and [[ GP IIb/IIa. 1 2 3 4 5 6 7 8 9 10  Arterial ]] and pathological levels of shear stress (>30 dynes/cm2) initiate platelet aggregation by inducing the binding of vWf to platelet GP Ib.	bind
19086	6	6128	7	NULL	NULL	NULL	NULL	statement 2	Process		requires					platelets	OrganismPart	metabolically active			NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_6_1399_s_18	7664419	1 2 3 4  5 6 7 8 9 10 14 15 16 17  The platelet aggregation response to fluid shear stress occurs in the absence of exogenous agonists 2  3  and requires intact vWf multimers, extracellular Ca2+, endogenous ADP contained in platelet granules, and metabolically active platelets with intact platelet membrane glycoprotein (GP) Ib and [[ GP IIb/IIa. 1 2 3 4 5 6 7 8 9 10  Arterial ]] and pathological levels of shear stress (>30 dynes/cm2) initiate platelet aggregation by inducing the binding of vWf to platelet GP Ib.	bind
19087	7	6128	7	NULL	NULL	NULL	NULL	platelets	OrganismPart	metabolically active	has intact					GP Ib	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_6_1399_s_18	7664419	1 2 3 4  5 6 7 8 9 10 14 15 16 17  The platelet aggregation response to fluid shear stress occurs in the absence of exogenous agonists 2  3  and requires intact vWf multimers, extracellular Ca2+, endogenous ADP contained in platelet granules, and metabolically active platelets with intact platelet membrane glycoprotein (GP) Ib and [[ GP IIb/IIa. 1 2 3 4 5 6 7 8 9 10  Arterial ]] and pathological levels of shear stress (>30 dynes/cm2) initiate platelet aggregation by inducing the binding of vWf to platelet GP Ib.	bind
19095	8	6128	7	NULL	NULL	NULL	NULL	shear stress	Process	pathological levels of	initiate					platelet 	OrganismPart	aggregation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_6_1399_s_18	7664419	1 2 3 4  5 6 7 8 9 10 14 15 16 17  The platelet aggregation response to fluid shear stress occurs in the absence of exogenous agonists 2  3  and requires intact vWf multimers, extracellular Ca2+, endogenous ADP contained in platelet granules, and metabolically active platelets with intact platelet membrane glycoprotein (GP) Ib and [[ GP IIb/IIa. 1 2 3 4 5 6 7 8 9 10  Arterial ]] and pathological levels of shear stress (>30 dynes/cm2) initiate platelet aggregation by inducing the binding of vWf to platelet GP Ib.	bind
19096	9	6128	7	NULL	NULL	NULL	NULL	statement 8	Process		occurs upon					statement 1	Process	inducing			NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_6_1399_s_18	7664419	1 2 3 4  5 6 7 8 9 10 14 15 16 17  The platelet aggregation response to fluid shear stress occurs in the absence of exogenous agonists 2  3  and requires intact vWf multimers, extracellular Ca2+, endogenous ADP contained in platelet granules, and metabolically active platelets with intact platelet membrane glycoprotein (GP) Ib and [[ GP IIb/IIa. 1 2 3 4 5 6 7 8 9 10  Arterial ]] and pathological levels of shear stress (>30 dynes/cm2) initiate platelet aggregation by inducing the binding of vWf to platelet GP Ib.	bind
45168	10	6128	7	NULL	NULL	NULL	NULL	GPIb	GP		is a type of					platelet membrane glycoprotein	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_6_1399_s_18	7664419	1 2 3 4  5 6 7 8 9 10 14 15 16 17  The platelet aggregation response to fluid shear stress occurs in the absence of exogenous agonists 2  3  and requires intact vWf multimers, extracellular Ca2+, endogenous ADP contained in platelet granules, and metabolically active platelets with intact platelet membrane glycoprotein (GP) Ib and [[ GP IIb/IIa. 1 2 3 4 5 6 7 8 9 10  Arterial ]] and pathological levels of shear stress (>30 dynes/cm2) initiate platelet aggregation by inducing the binding of vWf to platelet GP Ib.	bind
16072	1	6129	5	10	NULL	0	NULL	LDLs	NULL	binding of	is independent of	NULL				platelet	NULL	activation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_972_s_21	7541295	1 2 3 4  Binding of LDLs and HDLs was found to be independent of the state of platelet activation and was saturable.	bind
16073	2	6129	5	NULL	NULL	0	NULL	LDLs	NULL	binding of	is	NULL				saturable	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_972_s_21	7541295	1 2 3 4  Binding of LDLs and HDLs was found to be independent of the state of platelet activation and was saturable.	bind
16074	3	6129	5	10	NULL	0	NULL	HDLs	NULL	binding of	is independent of	NULL				platelet	NULL	activation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_972_s_21	7541295	1 2 3 4  Binding of LDLs and HDLs was found to be independent of the state of platelet activation and was saturable.	bind
16075	4	6129	5	NULL	NULL	0	NULL	HDLs	NULL	binding of	is	NULL				saturable	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_972_s_21	7541295	1 2 3 4  Binding of LDLs and HDLs was found to be independent of the state of platelet activation and was saturable.	bind
19097	1	6129	7	NULL	NULL	NULL	NULL	LDL	GP	binding of	independent of					platelet	OrganismPart	activation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_972_s_21	7541295	1 2 3 4  Binding of LDLs and HDLs was found to be independent of the state of platelet activation and was saturable.	bind
19098	2	6129	7	NULL	NULL	NULL	NULL	HDL	GP	binding of	independent of					platelet	OrganismPart	activation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_972_s_21	7541295	1 2 3 4  Binding of LDLs and HDLs was found to be independent of the state of platelet activation and was saturable.	bind
19099	3	6129	7	NULL	NULL	NULL	NULL	LDL	GP	binding of	is					saturable	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_972_s_21	7541295	1 2 3 4  Binding of LDLs and HDLs was found to be independent of the state of platelet activation and was saturable.	bind
19100	4	6129	7	NULL	NULL	NULL	NULL	HDL	GP	binding of	is					saturable	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_972_s_21	7541295	1 2 3 4  Binding of LDLs and HDLs was found to be independent of the state of platelet activation and was saturable.	bind
16076	1	6130	5	NULL	NULL	0	NULL	heparin	NULL		complex with	NULL				platelet factor 4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_14_1838_s_26	11294800	1 2 3 4  HIT is caused by the binding of antibodies (most frequently IgG) to a complex of heparin and platelet factor 4.	bind
16077	2	6130	5	NULL	NULL	0	NULL	IgG antibodies	NULL		bind	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_14_1838_s_26	11294800	1 2 3 4  HIT is caused by the binding of antibodies (most frequently IgG) to a complex of heparin and platelet factor 4.	bind
16078	3	6130	5	NULL	NULL	0	NULL	HIT	NULL		is caused by	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_14_1838_s_26	11294800	1 2 3 4  HIT is caused by the binding of antibodies (most frequently IgG) to a complex of heparin and platelet factor 4.	bind
19101	1	6130	7	NULL	NULL	NULL	NULL	heparin	GP		forms complex with					platelet factor 4	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_14_1838_s_26	11294800	1 2 3 4  HIT is caused by the binding of antibodies (most frequently IgG) to a complex of heparin and platelet factor 4.	bind
19102	2	6130	7	NULL	NULL	NULL	NULL	IgG	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_14_1838_s_26	11294800	1 2 3 4  HIT is caused by the binding of antibodies (most frequently IgG) to a complex of heparin and platelet factor 4.	bind
19103	3	6130	7	NULL	NULL	NULL	NULL	statement 2	Process		cause					HIT	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_14_1838_s_26	11294800	1 2 3 4  HIT is caused by the binding of antibodies (most frequently IgG) to a complex of heparin and platelet factor 4.	bind
16079	1	6133	5	10	NULL	0	NULL	growth factors	NULL	specific	bind	NULL				tyrosine kinases	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_19_1960_s_22	9609090	1 2 3 4 5  The binding of specific growth factors with their selective cell surface receptor tyrosine kinases results in its autophosphorylation and activation, leading to downstream signal transduction through chains of intercommunicating proteins culminating in cell proliferation.	bind
16080	2	6133	5	10	NULL	0	NULL	statement 1	NULL		results in	NULL				tyrosine kinases	NULL	autophosphorylation of 			NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_19_1960_s_22	9609090	1 2 3 4 5  The binding of specific growth factors with their selective cell surface receptor tyrosine kinases results in its autophosphorylation and activation, leading to downstream signal transduction through chains of intercommunicating proteins culminating in cell proliferation.	bind
16081	3	6133	5	10	NULL	0	NULL	statement 1	NULL		results in	NULL				tyrosine kinases	NULL	activation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_19_1960_s_22	9609090	1 2 3 4 5  The binding of specific growth factors with their selective cell surface receptor tyrosine kinases results in its autophosphorylation and activation, leading to downstream signal transduction through chains of intercommunicating proteins culminating in cell proliferation.	bind
24536	4	6133	5	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				signal transduction	NULL	downstream			NULL		0	NULL	NULL	NULL	gw60_circulation_97_19_1960_s_22	9609090	1 2 3 4 5  The binding of specific growth factors with their selective cell surface receptor tyrosine kinases results in its autophosphorylation and activation, leading to downstream signal transduction through chains of intercommunicating proteins culminating in cell proliferation.	bind
24537	5	6133	5	NULL	NULL	0	NULL	statement 4	NULL		occurs through	NULL				intercommunicating proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_97_19_1960_s_22	9609090	1 2 3 4 5  The binding of specific growth factors with their selective cell surface receptor tyrosine kinases results in its autophosphorylation and activation, leading to downstream signal transduction through chains of intercommunicating proteins culminating in cell proliferation.	bind
24538	6	6133	5	NULL	NULL	0	NULL	statement 5	NULL		results in	NULL				cell proliferation	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_97_19_1960_s_22	9609090	1 2 3 4 5  The binding of specific growth factors with their selective cell surface receptor tyrosine kinases results in its autophosphorylation and activation, leading to downstream signal transduction through chains of intercommunicating proteins culminating in cell proliferation.	bind
45200	7	6133	5	10	NULL	0	NULL	tyrosine kinase	NULL		is a type of	NULL				cell surface receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_97_19_1960_s_22	9609090	1 2 3 4 5  The binding of specific growth factors with their selective cell surface receptor tyrosine kinases results in its autophosphorylation and activation, leading to downstream signal transduction through chains of intercommunicating proteins culminating in cell proliferation.	bind
19106	1	6133	7	NULL	NULL	NULL	NULL	growth factors 	GP		bind					tyrosine kinases	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_19_1960_s_22	9609090	1 2 3 4 5  The binding of specific growth factors with their selective cell surface receptor tyrosine kinases results in its autophosphorylation and activation, leading to downstream signal transduction through chains of intercommunicating proteins culminating in cell proliferation.	bind
19107	2	6133	7	NULL	NULL	NULL	NULL	statement 1	Process		results in					tyrosine kinase	GP	autophosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_19_1960_s_22	9609090	1 2 3 4 5  The binding of specific growth factors with their selective cell surface receptor tyrosine kinases results in its autophosphorylation and activation, leading to downstream signal transduction through chains of intercommunicating proteins culminating in cell proliferation.	bind
19108	3	6133	7	NULL	NULL	NULL	NULL	statement 1	Process		results in					tyrosine kinase	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_19_1960_s_22	9609090	1 2 3 4 5  The binding of specific growth factors with their selective cell surface receptor tyrosine kinases results in its autophosphorylation and activation, leading to downstream signal transduction through chains of intercommunicating proteins culminating in cell proliferation.	bind
19109	4	6133	7	NULL	NULL	NULL	NULL	statement 2	Process		leads to					signal transduction	Process	downstream			NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_19_1960_s_22	9609090	1 2 3 4 5  The binding of specific growth factors with their selective cell surface receptor tyrosine kinases results in its autophosphorylation and activation, leading to downstream signal transduction through chains of intercommunicating proteins culminating in cell proliferation.	bind
19111	6	6133	7	NULL	NULL	NULL	NULL	signal transduction 	Process		occurs through					intercommunicating proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_19_1960_s_22	9609090	1 2 3 4 5  The binding of specific growth factors with their selective cell surface receptor tyrosine kinases results in its autophosphorylation and activation, leading to downstream signal transduction through chains of intercommunicating proteins culminating in cell proliferation.	bind
19112	7	6133	7	NULL	NULL	NULL	NULL	statement 6	Process		result in					cell profileration	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_19_1960_s_22	9609090	1 2 3 4 5  The binding of specific growth factors with their selective cell surface receptor tyrosine kinases results in its autophosphorylation and activation, leading to downstream signal transduction through chains of intercommunicating proteins culminating in cell proliferation.	bind
45201	8	6133	7	NULL	NULL	NULL	NULL	tyrosine kinase	GP		is a type of					cell surface receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_19_1960_s_22	9609090	1 2 3 4 5  The binding of specific growth factors with their selective cell surface receptor tyrosine kinases results in its autophosphorylation and activation, leading to downstream signal transduction through chains of intercommunicating proteins culminating in cell proliferation.	bind
16082	1	6134	5	NULL	NULL	0	NULL	heparin	NULL		bind	NULL				fibrin(ogen)	NULL	adsorbed			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_12_1948_s_21	9848889	1 2 Importantly, heparin binds to adsorbed fibrin(ogen) and prevents adhesion between fibrin-coated surfaces.	bind
16083	2	6134	5	NULL	NULL	0	NULL	statement 1	NULL		prevents	NULL				fibrin-coated surfaces	NULL	adhesion between			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_12_1948_s_21	9848889	1 2 Importantly, heparin binds to adsorbed fibrin(ogen) and prevents adhesion between fibrin-coated surfaces.	bind
19113	1	6134	7	NULL	NULL	NULL	NULL	heparin	GP		binds to					fibrinogen	GP	adsorbed			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_12_1948_s_21	9848889	1 2 Importantly, heparin binds to adsorbed fibrin(ogen) and prevents adhesion between fibrin-coated surfaces.	bind
19114	2	6134	7	NULL	NULL	NULL	NULL	statement 1	Process		prevents					fibrin-coated surfaces	GP	adhesion between			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_12_1948_s_21	9848889	1 2 Importantly, heparin binds to adsorbed fibrin(ogen) and prevents adhesion between fibrin-coated surfaces.	bind
16085	1	6135	5	10	NULL	0	NULL	norepinephrine	NULL		initiate	NULL				IP3 	NULL	signaling pathway of 			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_6_515_s_269	10488054	1 33  Furthermore, the observation that another agonist (norepinephrine) that binds to a different surface receptor than oxLDL but initiates the same IP3 signaling pathway as oxLDL also is incapable of generating a Ca2+ transient argues strongly that the primary defect is the IP3 signaling.	bind
16086	2	6135	5	NULL	NULL	0	NULL	statement 1	NULL		is incapable of 	NULL				Ca2+ transient	NULL	generating 			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_6_515_s_269	10488054	1 33  Furthermore, the observation that another agonist (norepinephrine) that binds to a different surface receptor than oxLDL but initiates the same IP3 signaling pathway as oxLDL also is incapable of generating a Ca2+ transient argues strongly that the primary defect is the IP3 signaling.	bind
16087	3	6135	5	NULL	NULL	0	NULL	statement 2	NULL		argues	NULL	strongly			IP3 	NULL	primary defect in signaling			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_6_515_s_269	10488054	1 33  Furthermore, the observation that another agonist (norepinephrine) that binds to a different surface receptor than oxLDL but initiates the same IP3 signaling pathway as oxLDL also is incapable of generating a Ca2+ transient argues strongly that the primary defect is the IP3 signaling.	bind
19115	1	6135	7	NULL	NULL	NULL	NULL	norepinephrine	Chemical		initiate					IP3	Chemical	signaling pathway of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_6_515_s_269	10488054	1 33  Furthermore, the observation that another agonist (norepinephrine) that binds to a different surface receptor than oxLDL but initiates the same IP3 signaling pathway as oxLDL also is incapable of generating a Ca2+ transient argues strongly that the primary defect is the IP3 signaling.	bind
19116	2	6135	7	NULL	NULL	NULL	NULL	norepinephrine	Chemical		is incapable of					Ca2+	Chemical	generating			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_6_515_s_269	10488054	1 33  Furthermore, the observation that another agonist (norepinephrine) that binds to a different surface receptor than oxLDL but initiates the same IP3 signaling pathway as oxLDL also is incapable of generating a Ca2+ transient argues strongly that the primary defect is the IP3 signaling.	bind
24172	3	6135	7	NULL	NULL	NULL	NULL	statement 3	Process		argues		strongly			IP3	Chemical	primary defect in signaling			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_6_515_s_269	10488054	1 33  Furthermore, the observation that another agonist (norepinephrine) that binds to a different surface receptor than oxLDL but initiates the same IP3 signaling pathway as oxLDL also is incapable of generating a Ca2+ transient argues strongly that the primary defect is the IP3 signaling.	bind
16088	1	6136	5	NULL	NULL	0	NULL	PU.1	NULL		bind	NULL				ganp	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_51_48000_s_155	11641399	1 Ab specifically inhibits binding of PU.1 to the  ganp promoter.	bind
16089	2	6136	5	NULL	NULL	0	NULL	Ab	NULL		inhibit	NULL	specifically			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_51_48000_s_155	11641399	1 Ab specifically inhibits binding of PU.1 to the  ganp promoter.	bind
19117	1	6136	7	NULL	NULL	NULL	NULL	PU.1	GP		bind					ganp	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_51_48000_s_155	11641399	1 Ab specifically inhibits binding of PU.1 to the  ganp promoter.	bind
19118	2	6136	7	NULL	NULL	NULL	NULL	Ab	GP		inhibits		specifically			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_51_48000_s_155	11641399	1 Ab specifically inhibits binding of PU.1 to the  ganp promoter.	bind
16090	1	6146	5	NULL	NULL	0	NULL	Ang1	NULL		is	NULL				Angiopoietin-1	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_139_2_329_s_2	12770938	1 Angiopoietin-1 (Ang1) is an angiogenic growth factor that binds to the Tie2 receptor on vascular endothelium, promoting blood vessel maturation and integrity.	bind
16091	2	6146	5	10	NULL	0	NULL	Ang1	NULL		bind	NULL				Tie2 receptor	NULL				NULL	on vascular endothelium	NULL	NULL	NULL	NULL	gw60_brjpharmacol_139_2_329_s_2	12770938	1 Angiopoietin-1 (Ang1) is an angiogenic growth factor that binds to the Tie2 receptor on vascular endothelium, promoting blood vessel maturation and integrity.	bind
16092	3	6146	5	NULL	NULL	0	NULL	statement 2	NULL		promotes	NULL				blood vessel	NULL	maturation of			NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_139_2_329_s_2	12770938	1 Angiopoietin-1 (Ang1) is an angiogenic growth factor that binds to the Tie2 receptor on vascular endothelium, promoting blood vessel maturation and integrity.	bind
16093	4	6146	5	NULL	NULL	0	NULL	statement 2	NULL		promotes	NULL				integrity	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_139_2_329_s_2	12770938	1 Angiopoietin-1 (Ang1) is an angiogenic growth factor that binds to the Tie2 receptor on vascular endothelium, promoting blood vessel maturation and integrity.	bind
45204	5	6146	5	10	NULL	0	NULL	Ang1	NULL		is a type of	NULL				angiogenic growth factor	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_139_2_329_s_2	12770938	1 Angiopoietin-1 (Ang1) is an angiogenic growth factor that binds to the Tie2 receptor on vascular endothelium, promoting blood vessel maturation and integrity.	bind
19119	1	6146	7	NULL	NULL	NULL	NULL	Ang1	GP		is a type of					angiogenic growth factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_139_2_329_s_2	12770938	1 Angiopoietin-1 (Ang1) is an angiogenic growth factor that binds to the Tie2 receptor on vascular endothelium, promoting blood vessel maturation and integrity.	bind
19120	2	6146	7	NULL	NULL	NULL	NULL	Ang1	GP		bind					Tie2 receptor	GP				NULL	vascular endothelium	NULL	NULL	NULL	NULL	gw60_brjpharmacol_139_2_329_s_2	12770938	1 Angiopoietin-1 (Ang1) is an angiogenic growth factor that binds to the Tie2 receptor on vascular endothelium, promoting blood vessel maturation and integrity.	bind
19121	3	6146	7	NULL	NULL	NULL	NULL	statement 2	Process		promotes					blood vessel	OrganismPart	maturation of			NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_139_2_329_s_2	12770938	1 Angiopoietin-1 (Ang1) is an angiogenic growth factor that binds to the Tie2 receptor on vascular endothelium, promoting blood vessel maturation and integrity.	bind
19122	4	6146	7	NULL	NULL	NULL	NULL	statement 2	Process		promotes					integrity	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_139_2_329_s_2	12770938	1 Angiopoietin-1 (Ang1) is an angiogenic growth factor that binds to the Tie2 receptor on vascular endothelium, promoting blood vessel maturation and integrity.	bind
19123	5	6146	7	NULL	NULL	NULL	NULL	Ang1	GP		is					Angiopoietin-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_139_2_329_s_2	12770938	1 Angiopoietin-1 (Ang1) is an angiogenic growth factor that binds to the Tie2 receptor on vascular endothelium, promoting blood vessel maturation and integrity.	bind
16094	1	6147	5	NULL	NULL	0	NULL	Sp1	NULL		bind	NULL				Sp1 probe	NULL	consensus			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_42_26236_s_233	9334192	1 antibody, unlike the anti-Sp1 antibody, failed to supershift Sp1 bound to a consensus Sp1 probe (Fig.  5 B, lanes 11-13).	bind
19124	1	6147	7	NULL	NULL	NULL	NULL	Sp1 	GP		bind					Sp1 probe	GP	consensus			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_42_26236_s_233	9334192	1 antibody, unlike the anti-Sp1 antibody, failed to supershift Sp1 bound to a consensus Sp1 probe (Fig.  5 B, lanes 11-13).	bind
16095	1	6148	5	NULL	NULL	0	NULL	Vitronectin	NULL		bind	NULL				Heparin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_11_6858_s_110	9054371	1 Binding of Vitronectin to Heparin Is Detected by Monitoring Changes in the Fluorescence of an Extrinsic Probe on Heparin	bind
19125	1	6148	7	NULL	NULL	NULL	NULL	Vitronectin	GP		bind					Heparin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_11_6858_s_110	9054371	1 Binding of Vitronectin to Heparin Is Detected by Monitoring Changes in the Fluorescence of an Extrinsic Probe on Heparin	bind
16096	1	6150	5	NULL	NULL	0	NULL	gp130	NULL		is	NULL				glycoprotein 130	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_12_1442_s_24	12234945	1 CT-1 binds to the glycoprotein 130 (gp130)/leukemia inhibitory factor (LIF) receptor complex 2 and activates both mitogen-activated protein kinase and janus kinase-signal transducer and activator of transcription (JAK-STAT) signaling pathways.	bind
16097	2	6150	5	NULL	NULL	0	NULL	LIF	NULL		is	NULL				leukemia inhibitory factor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_12_1442_s_24	12234945	1 CT-1 binds to the glycoprotein 130 (gp130)/leukemia inhibitory factor (LIF) receptor complex 2 and activates both mitogen-activated protein kinase and janus kinase-signal transducer and activator of transcription (JAK-STAT) signaling pathways.	bind
16098	3	6150	5	NULL	NULL	0	NULL	CT-1	NULL		bind	NULL				gp130/LIF receptor complex 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_12_1442_s_24	12234945	1 CT-1 binds to the glycoprotein 130 (gp130)/leukemia inhibitory factor (LIF) receptor complex 2 and activates both mitogen-activated protein kinase and janus kinase-signal transducer and activator of transcription (JAK-STAT) signaling pathways.	bind
16099	4	6150	5	NULL	NULL	0	NULL	statement 3	NULL		activates	NULL				mitogen-activated protein kinase	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_12_1442_s_24	12234945	1 CT-1 binds to the glycoprotein 130 (gp130)/leukemia inhibitory factor (LIF) receptor complex 2 and activates both mitogen-activated protein kinase and janus kinase-signal transducer and activator of transcription (JAK-STAT) signaling pathways.	bind
16100	5	6150	5	NULL	NULL	0	NULL	statement 3	NULL		activates	NULL				janus kinase-signal transducer	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_12_1442_s_24	12234945	1 CT-1 binds to the glycoprotein 130 (gp130)/leukemia inhibitory factor (LIF) receptor complex 2 and activates both mitogen-activated protein kinase and janus kinase-signal transducer and activator of transcription (JAK-STAT) signaling pathways.	bind
16101	6	6150	5	NULL	NULL	0	NULL	statement 3	NULL		activates	NULL				JAK-STAT signaling pathways	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_12_1442_s_24	12234945	1 CT-1 binds to the glycoprotein 130 (gp130)/leukemia inhibitory factor (LIF) receptor complex 2 and activates both mitogen-activated protein kinase and janus kinase-signal transducer and activator of transcription (JAK-STAT) signaling pathways.	bind
24539	7	6150	5	NULL	NULL	0	NULL	JAK-STAT signaling pathways	NULL		activates	NULL				transcription	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_12_1442_s_24	12234945	1 CT-1 binds to the glycoprotein 130 (gp130)/leukemia inhibitory factor (LIF) receptor complex 2 and activates both mitogen-activated protein kinase and janus kinase-signal transducer and activator of transcription (JAK-STAT) signaling pathways.	bind
19134	1	6150	7	NULL	NULL	NULL	NULL	CT-1	GP		binds to					gp130/LIF receptor complex 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_12_1442_s_24	12234945	1 CT-1 binds to the glycoprotein 130 (gp130)/leukemia inhibitory factor (LIF) receptor complex 2 and activates both mitogen-activated protein kinase and janus kinase-signal transducer and activator of transcription (JAK-STAT) signaling pathways.	bind
19135	2	6150	7	NULL	NULL	NULL	NULL	statement 1	Process		activates					mitogen-activated protein kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_12_1442_s_24	12234945	1 CT-1 binds to the glycoprotein 130 (gp130)/leukemia inhibitory factor (LIF) receptor complex 2 and activates both mitogen-activated protein kinase and janus kinase-signal transducer and activator of transcription (JAK-STAT) signaling pathways.	bind
19136	3	6150	7	NULL	NULL	NULL	NULL	statement 1	Process		activates					janus kinase-signal transducer	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_12_1442_s_24	12234945	1 CT-1 binds to the glycoprotein 130 (gp130)/leukemia inhibitory factor (LIF) receptor complex 2 and activates both mitogen-activated protein kinase and janus kinase-signal transducer and activator of transcription (JAK-STAT) signaling pathways.	bind
19137	4	6150	7	NULL	NULL	NULL	NULL	statement 1	Process		activates					JAK-STAT signaling pathway	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_12_1442_s_24	12234945	1 CT-1 binds to the glycoprotein 130 (gp130)/leukemia inhibitory factor (LIF) receptor complex 2 and activates both mitogen-activated protein kinase and janus kinase-signal transducer and activator of transcription (JAK-STAT) signaling pathways.	bind
19138	5	6150	7	NULL	NULL	NULL	NULL	gp130	GP		is					glycoprotein 130	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_12_1442_s_24	12234945	1 CT-1 binds to the glycoprotein 130 (gp130)/leukemia inhibitory factor (LIF) receptor complex 2 and activates both mitogen-activated protein kinase and janus kinase-signal transducer and activator of transcription (JAK-STAT) signaling pathways.	bind
19139	6	6150	7	NULL	NULL	NULL	NULL	LIF	GP		is					leukemia inhibitory factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_12_1442_s_24	12234945	1 CT-1 binds to the glycoprotein 130 (gp130)/leukemia inhibitory factor (LIF) receptor complex 2 and activates both mitogen-activated protein kinase and janus kinase-signal transducer and activator of transcription (JAK-STAT) signaling pathways.	bind
19140	7	6150	7	NULL	NULL	NULL	NULL	JAK-STAT pathway	Process		activates					transcription	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_12_1442_s_24	12234945	1 CT-1 binds to the glycoprotein 130 (gp130)/leukemia inhibitory factor (LIF) receptor complex 2 and activates both mitogen-activated protein kinase and janus kinase-signal transducer and activator of transcription (JAK-STAT) signaling pathways.	bind
16102	1	6151	5	10	NULL	0	NULL	Vps45	NULL		bind	NULL	differential			Tlg2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1641_2_111_s_718	12914952	1 Differential binding of SM protein Vps45 to Tlg2 has recently suggested by N.J. Bryant  and D.E. James, J. Cell Biol. 161 (2003) 691-696.	bind
45205	2	6151	5	10	NULL	0	NULL	Vps45	NULL		is a type of	NULL				SM protein	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1641_2_111_s_718	12914952	1 Differential binding of SM protein Vps45 to Tlg2 has recently suggested by N.J. Bryant  and D.E. James, J. Cell Biol. 161 (2003) 691-696.	bind
19141	1	6151	7	NULL	NULL	NULL	NULL	Vps45	GP		bind		differentially			Tlg2	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1641_2_111_s_718	12914952	1 Differential binding of SM protein Vps45 to Tlg2 has recently suggested by N.J. Bryant  and D.E. James, J. Cell Biol. 161 (2003) 691-696.	bind
45206	2	6151	7	NULL	NULL	NULL	NULL	Vps45	GP		is a type of					SM protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1641_2_111_s_718	12914952	1 Differential binding of SM protein Vps45 to Tlg2 has recently suggested by N.J. Bryant  and D.E. James, J. Cell Biol. 161 (2003) 691-696.	bind
16104	1	6154	5	NULL	NULL	0	NULL	PU.1	NULL		is necessary for	NULL		Ets DNA binding domain		nuclear localization	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_11_10675_s_4	15632149	1 fusions, we show that the Ets DNA binding domain of PU.1 is necessary and sufficient for its nuclear localization.	bind
16106	2	6154	5	NULL	NULL	0	NULL	PU.1	NULL		is sufficient for	NULL		Ets DNA binding domain		nuclear localization	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_11_10675_s_4	15632149	1 fusions, we show that the Ets DNA binding domain of PU.1 is necessary and sufficient for its nuclear localization.	bind
19142	1	6154	7	NULL	NULL	NULL	NULL	PU.1	GP		is necessary for			Ets DNA binding domain		nuclear localization	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_10675_s_4	15632149	1 fusions, we show that the Ets DNA binding domain of PU.1 is necessary and sufficient for its nuclear localization.	bind
19143	2	6154	7	NULL	NULL	NULL	NULL	PU.1	GP		sufficient for			Ets DNA binding domain		nuclear localization	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_10675_s_4	15632149	1 fusions, we show that the Ets DNA binding domain of PU.1 is necessary and sufficient for its nuclear localization.	bind
16107	1	6155	5	NULL	NULL	0	NULL	GT335 IgGs	NULL		bind	NULL				tubulin	NULL	brain			NULL		0	NULL	NULL	NULL	gw60_cellbiol_143_6_1575_s_81	9852152	1 immunoglobulins were prepared by the caprylic acid method, and GT335 IgGs  were affinity-purified on brain tubulin bound to a Hi-Trap column ( Pharmacia Biotech, Piscataway, NJ).	bind
19144	1	6155	7	NULL	NULL	NULL	NULL	GT335 IgGs	GP		bind					tubulin	GP	brain			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_143_6_1575_s_81	9852152	1 immunoglobulins were prepared by the caprylic acid method, and GT335 IgGs  were affinity-purified on brain tubulin bound to a Hi-Trap column ( Pharmacia Biotech, Piscataway, NJ).	bind
16108	1	6156	5	NULL	NULL	0	NULL	Munc18-1	NULL		bind	NULL	strongly			syntaxin 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_50_31459_s_22	9395480	1 In addition to binding strongly to syntaxin 1, Munc18-1 binds to Doc2a and Doc2b, C2 domain proteins that are associated peripherally with synaptic vesicles ( 10).	bind
16109	2	6156	5	NULL	NULL	0	NULL	Munc18-1	NULL		bind	NULL				Doc2a	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_50_31459_s_22	9395480	1 In addition to binding strongly to syntaxin 1, Munc18-1 binds to Doc2a and Doc2b, C2 domain proteins that are associated peripherally with synaptic vesicles ( 10).	bind
16110	3	6156	5	NULL	NULL	0	NULL	Munc18-1	NULL		bind	NULL				Doc2a	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_50_31459_s_22	9395480	1 In addition to binding strongly to syntaxin 1, Munc18-1 binds to Doc2a and Doc2b, C2 domain proteins that are associated peripherally with synaptic vesicles ( 10).	bind
16111	4	6156	5	NULL	NULL	0	NULL	C2 domain proteins	NULL		associate with	NULL	peripherally			synaptic vesicles	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31459_s_22	9395480	1 In addition to binding strongly to syntaxin 1, Munc18-1 binds to Doc2a and Doc2b, C2 domain proteins that are associated peripherally with synaptic vesicles ( 10).	bind
16112	5	6156	5	NULL	NULL	0	NULL	Munc18-1	NULL		bind	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_50_31459_s_22	9395480	1 In addition to binding strongly to syntaxin 1, Munc18-1 binds to Doc2a and Doc2b, C2 domain proteins that are associated peripherally with synaptic vesicles ( 10).	bind
24540	6	6156	5	NULL	NULL	0	NULL	Doc2a	NULL		associate with	NULL	peripherally			synaptic vesicles	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31459_s_22	9395480	1 In addition to binding strongly to syntaxin 1, Munc18-1 binds to Doc2a and Doc2b, C2 domain proteins that are associated peripherally with synaptic vesicles ( 10).	bind
24541	7	6156	5	NULL	NULL	0	NULL	Doc2b	NULL		associate with	NULL	peripherally			synaptic vesicles	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_50_31459_s_22	9395480	1 In addition to binding strongly to syntaxin 1, Munc18-1 binds to Doc2a and Doc2b, C2 domain proteins that are associated peripherally with synaptic vesicles ( 10).	bind
19145	1	6156	7	NULL	NULL	NULL	NULL	Munc18-1	GP		binds to					Doc2a	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31459_s_22	9395480	1 In addition to binding strongly to syntaxin 1, Munc18-1 binds to Doc2a and Doc2b, C2 domain proteins that are associated peripherally with synaptic vesicles ( 10).	bind
19146	2	6156	7	NULL	NULL	NULL	NULL	Munc18-1	GP		binds to					Doc2b	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31459_s_22	9395480	1 In addition to binding strongly to syntaxin 1, Munc18-1 binds to Doc2a and Doc2b, C2 domain proteins that are associated peripherally with synaptic vesicles ( 10).	bind
19148	3	6156	7	NULL	NULL	NULL	NULL	Munc18-1	GP		binds to		strongly			syntaxin 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31459_s_22	9395480	1 In addition to binding strongly to syntaxin 1, Munc18-1 binds to Doc2a and Doc2b, C2 domain proteins that are associated peripherally with synaptic vesicles ( 10).	bind
19149	4	6156	7	NULL	NULL	NULL	NULL	Doc2a	GP		associate with		peripherally			synaptic vesicles	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31459_s_22	9395480	1 In addition to binding strongly to syntaxin 1, Munc18-1 binds to Doc2a and Doc2b, C2 domain proteins that are associated peripherally with synaptic vesicles ( 10).	bind
19150	5	6156	7	NULL	NULL	NULL	NULL	Doc2b	GP		associate with		peripherally			synaptic vesicles	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31459_s_22	9395480	1 In addition to binding strongly to syntaxin 1, Munc18-1 binds to Doc2a and Doc2b, C2 domain proteins that are associated peripherally with synaptic vesicles ( 10).	bind
19151	6	6156	7	NULL	NULL	NULL	NULL	C2 domain proteins	GP		associate with		peripherally			synaptic vesicles	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31459_s_22	9395480	1 In addition to binding strongly to syntaxin 1, Munc18-1 binds to Doc2a and Doc2b, C2 domain proteins that are associated peripherally with synaptic vesicles ( 10).	bind
24173	7	6156	7	NULL	NULL	NULL	NULL	Munc18-1	GP		bind					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31459_s_22	9395480	1 In addition to binding strongly to syntaxin 1, Munc18-1 binds to Doc2a and Doc2b, C2 domain proteins that are associated peripherally with synaptic vesicles ( 10).	bind
16113	1	6157	5	NULL	NULL	0	NULL	Netrin	NULL		bind	NULL				receptor Unc5b	NULL				NULL	in vascular system of fish	0	NULL	NULL	NULL	gw70_circulationres_98_4_440_s_20	16514073	1 In the vascular system of fish and mice, Netrin binding to the receptor Unc5b suppresses the formation of endothelial tip cell filopodia and branching of blood vessels.	bind
16114	2	6157	5	NULL	NULL	0	NULL	Netrin	NULL		bind	NULL				receptor Unc5b	NULL				NULL	in vascular system of mice	0	NULL	NULL	NULL	gw70_circulationres_98_4_440_s_20	16514073	1 In the vascular system of fish and mice, Netrin binding to the receptor Unc5b suppresses the formation of endothelial tip cell filopodia and branching of blood vessels.	bind
16115	3	6157	5	10	NULL	0	NULL	statement 1			supress					endothelial tip cell filopodia		formation of 			NULL	vascular system of fish	NULL	NULL	NULL	NULL	gw70_circulationres_98_4_440_s_20	16514073	1 In the vascular system of fish and mice, Netrin binding to the receptor Unc5b suppresses the formation of endothelial tip cell filopodia and branching of blood vessels.	bind
16116	4	6157	5	10	NULL	0	NULL	statement 2			supress					endothelial tip cell filopodia		formation of			NULL	vascular system of mice	NULL	NULL	NULL	NULL	gw70_circulationres_98_4_440_s_20	16514073	1 In the vascular system of fish and mice, Netrin binding to the receptor Unc5b suppresses the formation of endothelial tip cell filopodia and branching of blood vessels.	bind
16118	5	6157	5	10	NULL	0	NULL	statement 1			supress					blood vessels		branching of 			NULL	vascular system of fish	NULL	NULL	NULL	NULL	gw70_circulationres_98_4_440_s_20	16514073	1 In the vascular system of fish and mice, Netrin binding to the receptor Unc5b suppresses the formation of endothelial tip cell filopodia and branching of blood vessels.	bind
16120	6	6157	5	10	NULL	0	NULL	statement 2			supress					blood vessels		branching of			NULL	vascular system of mice	NULL	NULL	NULL	NULL	gw70_circulationres_98_4_440_s_20	16514073	1 In the vascular system of fish and mice, Netrin binding to the receptor Unc5b suppresses the formation of endothelial tip cell filopodia and branching of blood vessels.	bind
19154	1	6157	7	NULL	NULL	NULL	NULL	Netrin	GP		bind					Unc5b receptor	GP				NULL	vascular system of fish	NULL	NULL	NULL	NULL	gw70_circulationres_98_4_440_s_20	16514073	1 In the vascular system of fish and mice, Netrin binding to the receptor Unc5b suppresses the formation of endothelial tip cell filopodia and branching of blood vessels.	bind
19155	2	6157	7	NULL	NULL	NULL	NULL	Netrin	GP		bind					Unc5b receptor	GP				NULL	vascular system of mice	NULL	NULL	NULL	NULL	gw70_circulationres_98_4_440_s_20	16514073	1 In the vascular system of fish and mice, Netrin binding to the receptor Unc5b suppresses the formation of endothelial tip cell filopodia and branching of blood vessels.	bind
19156	3	6157	7	NULL	NULL	NULL	NULL	statement 1	Process		suppress					endothelial tip cell filopodia	OrganismPart	formation of			NULL	vascular system of fish	NULL	NULL	NULL	NULL	gw70_circulationres_98_4_440_s_20	16514073	1 In the vascular system of fish and mice, Netrin binding to the receptor Unc5b suppresses the formation of endothelial tip cell filopodia and branching of blood vessels.	bind
19157	4	6157	7	NULL	NULL	NULL	NULL	statement 1	Process		suppress					blood vessel	OrganismPart	branching of			NULL	vascular system of fish	NULL	NULL	NULL	NULL	gw70_circulationres_98_4_440_s_20	16514073	1 In the vascular system of fish and mice, Netrin binding to the receptor Unc5b suppresses the formation of endothelial tip cell filopodia and branching of blood vessels.	bind
19158	5	6157	7	NULL	NULL	NULL	NULL	statement 2	Process		suppress					endothelial tip cell filopodia	OrganismPart	formation of			NULL	vascular system of mice	NULL	NULL	NULL	NULL	gw70_circulationres_98_4_440_s_20	16514073	1 In the vascular system of fish and mice, Netrin binding to the receptor Unc5b suppresses the formation of endothelial tip cell filopodia and branching of blood vessels.	bind
19159	6	6157	7	NULL	NULL	NULL	NULL	statement 2	Process		suppress					blood vessel	OrganismPart	branching of			NULL	vascular system of mice	NULL	NULL	NULL	NULL	gw70_circulationres_98_4_440_s_20	16514073	1 In the vascular system of fish and mice, Netrin binding to the receptor Unc5b suppresses the formation of endothelial tip cell filopodia and branching of blood vessels.	bind
16122	1	6159	5	NULL	NULL	0	NULL	TfRs	NULL		is	NULL				Tf receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_46_33035_s_16	10551872	1 Iron uptake from Tf involves the binding of Tf to the Tf receptors (TfRs), internalization of Tf within an endocytic vesicle by receptor-mediated endocytosis, and the release of iron from Tf by a decrease in endosomal pH.	bind
16124	2	6159	5	NULL	NULL	0	NULL	TfRs	NULL		bind	NULL				TfRs	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_46_33035_s_16	10551872	1 Iron uptake from Tf involves the binding of Tf to the Tf receptors (TfRs), internalization of Tf within an endocytic vesicle by receptor-mediated endocytosis, and the release of iron from Tf by a decrease in endosomal pH.	bind
16125	3	6159	5	NULL	NULL	0	NULL	Tf	NULL	iron uptake from	involves	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_46_33035_s_16	10551872	1 Iron uptake from Tf involves the binding of Tf to the Tf receptors (TfRs), internalization of Tf within an endocytic vesicle by receptor-mediated endocytosis, and the release of iron from Tf by a decrease in endosomal pH.	bind
16127	4	6159	5	NULL	NULL	0	NULL	Tf	NULL		is internalized within	NULL				endocytic vesicle	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_46_33035_s_16	10551872	1 Iron uptake from Tf involves the binding of Tf to the Tf receptors (TfRs), internalization of Tf within an endocytic vesicle by receptor-mediated endocytosis, and the release of iron from Tf by a decrease in endosomal pH.	bind
16128	6	6159	5	NULL	NULL	0	NULL	Tf	NULL	iron uptake from	involves	NULL				statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_46_33035_s_16	10551872	1 Iron uptake from Tf involves the binding of Tf to the Tf receptors (TfRs), internalization of Tf within an endocytic vesicle by receptor-mediated endocytosis, and the release of iron from Tf by a decrease in endosomal pH.	bind
16129	7	6159	5	NULL	NULL	0	NULL	iron	NULL		released from	NULL				Tf	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_46_33035_s_16	10551872	1 Iron uptake from Tf involves the binding of Tf to the Tf receptors (TfRs), internalization of Tf within an endocytic vesicle by receptor-mediated endocytosis, and the release of iron from Tf by a decrease in endosomal pH.	bind
16130	8	6159	5	NULL	NULL	0	NULL	endosomal pH	NULL	decrease in	leads to	NULL				statement 7	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_46_33035_s_16	10551872	1 Iron uptake from Tf involves the binding of Tf to the Tf receptors (TfRs), internalization of Tf within an endocytic vesicle by receptor-mediated endocytosis, and the release of iron from Tf by a decrease in endosomal pH.	bind
16131	9	6159	5	NULL	NULL	0	NULL	Tf	NULL	iron uptake from	involves	NULL				statement 8	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_46_33035_s_16	10551872	1 Iron uptake from Tf involves the binding of Tf to the Tf receptors (TfRs), internalization of Tf within an endocytic vesicle by receptor-mediated endocytosis, and the release of iron from Tf by a decrease in endosomal pH.	bind
16134	5	6159	5	NULL	NULL	0	NULL	endocytosis	NULL	receptor-mediated	leads to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_46_33035_s_16	10551872	1 Iron uptake from Tf involves the binding of Tf to the Tf receptors (TfRs), internalization of Tf within an endocytic vesicle by receptor-mediated endocytosis, and the release of iron from Tf by a decrease in endosomal pH.	bind
20793	1	6159	7	NULL	NULL	NULL	NULL	Tf	GP		bind					TfRs	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_46_33035_s_16	10551872	1 Iron uptake from Tf involves the binding of Tf to the Tf receptors (TfRs), internalization of Tf within an endocytic vesicle by receptor-mediated endocytosis, and the release of iron from Tf by a decrease in endosomal pH.	bind
20794	2	6159	7	NULL	NULL	NULL	NULL	Tf	GP	Iron uptake from	involves					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_46_33035_s_16	10551872	1 Iron uptake from Tf involves the binding of Tf to the Tf receptors (TfRs), internalization of Tf within an endocytic vesicle by receptor-mediated endocytosis, and the release of iron from Tf by a decrease in endosomal pH.	bind
20797	3	6159	7	NULL	NULL	NULL	NULL	endocytosis	Process	 receptor-mediated	internalize					Tf	GP	within endocytic vesicle 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_46_33035_s_16	10551872	1 Iron uptake from Tf involves the binding of Tf to the Tf receptors (TfRs), internalization of Tf within an endocytic vesicle by receptor-mediated endocytosis, and the release of iron from Tf by a decrease in endosomal pH.	bind
20798	4	6159	7	NULL	NULL	NULL	NULL	Tf	GP	Iron uptake from	involves					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_46_33035_s_16	10551872	1 Iron uptake from Tf involves the binding of Tf to the Tf receptors (TfRs), internalization of Tf within an endocytic vesicle by receptor-mediated endocytosis, and the release of iron from Tf by a decrease in endosomal pH.	bind
20802	5	6159	7	NULL	NULL	NULL	NULL	pH	QuantityOrMeasure	decrease in endosomal	release					Tf	GP	iron from			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_46_33035_s_16	10551872	1 Iron uptake from Tf involves the binding of Tf to the Tf receptors (TfRs), internalization of Tf within an endocytic vesicle by receptor-mediated endocytosis, and the release of iron from Tf by a decrease in endosomal pH.	bind
20813	6	6159	7	NULL	NULL	NULL	NULL	Tf	GP	Iron uptake from	involves					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_46_33035_s_16	10551872	1 Iron uptake from Tf involves the binding of Tf to the Tf receptors (TfRs), internalization of Tf within an endocytic vesicle by receptor-mediated endocytosis, and the release of iron from Tf by a decrease in endosomal pH.	bind
20814	7	6159	7	NULL	NULL	NULL	NULL	TfRs	GP		is					Tf receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_46_33035_s_16	10551872	1 Iron uptake from Tf involves the binding of Tf to the Tf receptors (TfRs), internalization of Tf within an endocytic vesicle by receptor-mediated endocytosis, and the release of iron from Tf by a decrease in endosomal pH.	bind
16135	1	6160	5	NULL	NULL	0	NULL	ERNS antibodies	NULL		bind	NULL				ERNS antigen	NULL				NULL		0	NULL	NULL	NULL	gw60_vetmicrobiol_73_2_209_s_112	10785329	1 is conjugated with HRPO and used for detection of binding of ERNS antibodies to the ERNS antigen.	bind
20822	1	6160	7	NULL	NULL	NULL	NULL	ERNS antibodies	GP		bind					ERNS antigen	GP				NULL		NULL	NULL	NULL	NULL	gw60_vetmicrobiol_73_2_209_s_112	10785329	1 is conjugated with HRPO and used for detection of binding of ERNS antibodies to the ERNS antigen.	bind
16473	1	6162	5	NULL	NULL	0	NULL	phage-antibodies	NULL		bind	NULL				microcystin-LR-BSA conjugates	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_11_5288_s_128	12406716	1 library prior to affinity selection (pan 0) and from each subsequent pan indicated an enrichment of phage-antibodies which bound to microcystin-LR-BSA and microcystin-LR-KLH conjugates (Fig.  1).	bind
16474	2	6162	5	NULL	NULL	0	NULL	phage-antibodies	NULL		bind	NULL				microcystin-LR-KLH conjugates	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_11_5288_s_128	12406716	1 library prior to affinity selection (pan 0) and from each subsequent pan indicated an enrichment of phage-antibodies which bound to microcystin-LR-BSA and microcystin-LR-KLH conjugates (Fig.  1).	bind
20827	1	6162	7	NULL	NULL	NULL	NULL	phage-antibodies	GP		bind					microcystin-LR-BSA conjugate	GP				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_68_11_5288_s_128	12406716	1 library prior to affinity selection (pan 0) and from each subsequent pan indicated an enrichment of phage-antibodies which bound to microcystin-LR-BSA and microcystin-LR-KLH conjugates (Fig.  1).	bind
20828	2	6162	7	NULL	NULL	NULL	NULL	phage-antibodies	GP		bind					microcystin-LR-KLH conjugate	GP				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_68_11_5288_s_128	12406716	1 library prior to affinity selection (pan 0) and from each subsequent pan indicated an enrichment of phage-antibodies which bound to microcystin-LR-BSA and microcystin-LR-KLH conjugates (Fig.  1).	bind
16475	1	6163	5	NULL	NULL	0	NULL	CRP	NULL	aggregated	bind	NULL				C1q	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_17_2019_s_19	11980679	1 Ligand-bound or aggregated CRP binds C1q and in so doing activates the classical complement pathway.	bind
16476	2	6163	5	NULL	NULL	0	NULL	statement 1	NULL		activates	NULL				classical complement pathway	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_17_2019_s_19	11980679	1 Ligand-bound or aggregated CRP binds C1q and in so doing activates the classical complement pathway.	bind
16477	3	6163	5	NULL	NULL	0	NULL	CRP	NULL	ligand-bound	bind	NULL				C1q	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_17_2019_s_19	11980679	1 Ligand-bound or aggregated CRP binds C1q and in so doing activates the classical complement pathway.	bind
16478	4	6163	5	NULL	NULL	0	NULL	statement 3	NULL		activates	NULL				classical complement pathway	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_17_2019_s_19	11980679	1 Ligand-bound or aggregated CRP binds C1q and in so doing activates the classical complement pathway.	bind
20829	1	6163	7	NULL	NULL	NULL	NULL	CRP	GP	Ligand-bound	binds					C1q	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_17_2019_s_19	11980679	1 Ligand-bound or aggregated CRP binds C1q and in so doing activates the classical complement pathway.	bind
20830	2	6163	7	NULL	NULL	NULL	NULL	CRP	GP	aggregated	binds					C1q	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_17_2019_s_19	11980679	1 Ligand-bound or aggregated CRP binds C1q and in so doing activates the classical complement pathway.	bind
20831	3	6163	7	NULL	NULL	NULL	NULL	statement 1	Process		activates					classical complement pathway	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_17_2019_s_19	11980679	1 Ligand-bound or aggregated CRP binds C1q and in so doing activates the classical complement pathway.	bind
20832	4	6163	7	NULL	NULL	NULL	NULL	statement 2	Process		activates					classical complement pathway	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_17_2019_s_19	11980679	1 Ligand-bound or aggregated CRP binds C1q and in so doing activates the classical complement pathway.	bind
16479	1	6167	5	NULL	NULL	0	NULL	MRP-8/14 complex	NULL	native	bind	NULL				CHO-K1 cells	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_5_3658_s_198	11723110	1 muM native MRP-8/14 complex binding to CHO-K1 ( ) and pgsA-745 cells ( ) as detected by anti-MRP-14.	bind
16480	2	6167	5	NULL	NULL	0	NULL	MRP-8/14 complex	NULL	native	bind	NULL				pgsA-745 cells	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_5_3658_s_198	11723110	1 muM native MRP-8/14 complex binding to CHO-K1 ( ) and pgsA-745 cells ( ) as detected by anti-MRP-14.	bind
20833	1	6167	7	NULL	NULL	NULL	NULL	MRP-8/14 complex	GP	native	bind					CHO-K1 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_5_3658_s_198	11723110	1 muM native MRP-8/14 complex binding to CHO-K1 ( ) and pgsA-745 cells ( ) as detected by anti-MRP-14.	bind
20834	2	6167	7	NULL	NULL	NULL	NULL	MRP-8/14 complex	GP	native	bind					pgsA-745 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_5_3658_s_198	11723110	1 muM native MRP-8/14 complex binding to CHO-K1 ( ) and pgsA-745 cells ( ) as detected by anti-MRP-14.	bind
24542	1	6169	5	NULL	NULL	0	NULL	SHP	NULL		contains	NULL					NULL		two N terminus SH2 domains		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_6_3687_s_12	9452499	1 One subfamily of cytoplasmic PTPs, referred to as SHP ( 1), contains two SH2 domains at their N terminus.	bind
24543	2	6169	5	NULL	NULL	0	NULL	SHP	NULL		is a subfamily of	NULL				cytoplasmic PTPs	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_6_3687_s_12	9452499	1 One subfamily of cytoplasmic PTPs, referred to as SHP ( 1), contains two SH2 domains at their N terminus.	bind
20835	1	6169	7	NULL	NULL	NULL	NULL	SHP	GP		contains								2 N terminus SH2 domains		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_6_3687_s_12	9452499	1 One subfamily of cytoplasmic PTPs, referred to as SHP ( 1), contains two SH2 domains at their N terminus.	bind
20836	2	6169	7	NULL	NULL	NULL	NULL	SHP	GP		is a subfamily of					cytoplasmic PTPs	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_6_3687_s_12	9452499	1 One subfamily of cytoplasmic PTPs, referred to as SHP ( 1), contains two SH2 domains at their N terminus.	bind
16481	1	6170	5	NULL	NULL	0	NULL	EGF-like ligands	NULL	mammalian	include	NULL				TGFalpha	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_138_4_747_s_13	9265643	1 Other mammalian EGF-like ligands include transforming growth factor-alpha (TGFalpha), amphiregulin, heparin binding EGF-like  growth factor, betacellulin and epiregulin ( 3,  17,  32).	bind
16482	2	6170	5	NULL	NULL	0	NULL	TGFalpha	NULL		is	NULL				transforming growth factor-alpha	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_138_4_747_s_13	9265643	1 Other mammalian EGF-like ligands include transforming growth factor-alpha (TGFalpha), amphiregulin, heparin binding EGF-like  growth factor, betacellulin and epiregulin ( 3,  17,  32).	bind
16483	3	6170	5	NULL	NULL	0	NULL	EGF-like ligands	NULL	mammalian	include	NULL				amphiregulin	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_138_4_747_s_13	9265643	1 Other mammalian EGF-like ligands include transforming growth factor-alpha (TGFalpha), amphiregulin, heparin binding EGF-like  growth factor, betacellulin and epiregulin ( 3,  17,  32).	bind
16484	4	6170	5	NULL	NULL	0	NULL	EGF-like ligands	NULL	mammalian	include	NULL				EGF-like growth factor	NULL	heparin binding			NULL		0	NULL	NULL	NULL	gw60_cellbiol_138_4_747_s_13	9265643	1 Other mammalian EGF-like ligands include transforming growth factor-alpha (TGFalpha), amphiregulin, heparin binding EGF-like  growth factor, betacellulin and epiregulin ( 3,  17,  32).	bind
16485	5	6170	5	NULL	NULL	0	NULL	EGF-like ligands	NULL	mammalian	include	NULL				betacellulin	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_138_4_747_s_13	9265643	1 Other mammalian EGF-like ligands include transforming growth factor-alpha (TGFalpha), amphiregulin, heparin binding EGF-like  growth factor, betacellulin and epiregulin ( 3,  17,  32).	bind
16486	6	6170	5	NULL	NULL	0	NULL	EGF-like ligands	NULL	mammalian	include	NULL				epiregulin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_138_4_747_s_13	9265643	1 Other mammalian EGF-like ligands include transforming growth factor-alpha (TGFalpha), amphiregulin, heparin binding EGF-like  growth factor, betacellulin and epiregulin ( 3,  17,  32).	bind
20837	1	6170	7	NULL	NULL	NULL	NULL	EGF-like ligands	GP	mammalian	include					TGFalpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_138_4_747_s_13	9265643	1 Other mammalian EGF-like ligands include transforming growth factor-alpha (TGFalpha), amphiregulin, heparin binding EGF-like  growth factor, betacellulin and epiregulin ( 3,  17,  32).	bind
20838	2	6170	7	NULL	NULL	NULL	NULL	EGF-like ligands	GP	mammalian	include					amphiregulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_138_4_747_s_13	9265643	1 Other mammalian EGF-like ligands include transforming growth factor-alpha (TGFalpha), amphiregulin, heparin binding EGF-like  growth factor, betacellulin and epiregulin ( 3,  17,  32).	bind
20839	3	6170	7	NULL	NULL	NULL	NULL	EGF-like ligands	GP	mammalian	include					EGF-like growth factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_138_4_747_s_13	9265643	1 Other mammalian EGF-like ligands include transforming growth factor-alpha (TGFalpha), amphiregulin, heparin binding EGF-like  growth factor, betacellulin and epiregulin ( 3,  17,  32).	bind
20840	4	6170	7	NULL	NULL	NULL	NULL	EGF-like ligands	GP	mammalian	include					betacellulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_138_4_747_s_13	9265643	1 Other mammalian EGF-like ligands include transforming growth factor-alpha (TGFalpha), amphiregulin, heparin binding EGF-like  growth factor, betacellulin and epiregulin ( 3,  17,  32).	bind
20841	5	6170	7	NULL	NULL	NULL	NULL	EGF-like ligands	GP	mammalian	include					epiregulin 	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_138_4_747_s_13	9265643	1 Other mammalian EGF-like ligands include transforming growth factor-alpha (TGFalpha), amphiregulin, heparin binding EGF-like  growth factor, betacellulin and epiregulin ( 3,  17,  32).	bind
24174	6	6170	7	NULL	NULL	NULL	NULL	TGFalpha	GP		is					transforming growth factor-alpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_138_4_747_s_13	9265643	1 Other mammalian EGF-like ligands include transforming growth factor-alpha (TGFalpha), amphiregulin, heparin binding EGF-like  growth factor, betacellulin and epiregulin ( 3,  17,  32).	bind
55019	7	6170	7	NULL	NULL	NULL	NULL	EGF-like growth factor	GP		bind					heparin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_138_4_747_s_13	9265643	1 Other mammalian EGF-like ligands include transforming growth factor-alpha (TGFalpha), amphiregulin, heparin binding EGF-like  growth factor, betacellulin and epiregulin ( 3,  17,  32).	bind
16487	1	6171	5	NULL	NULL	0	NULL	IRSs	NULL	phosphorylated	bind	NULL				enzymes	NULL		SH2 domain		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_28_25323_s_11	12730241	1 Phosphorylated IRSs bind and activate SH2 domain enzymes to couple the  activated receptors to such downstream metabolic effects as glucose uptake and  glycogen and triglyceride synthesis and storage.	bind
16488	2	6171	5	NULL	NULL	0	NULL	IRSs	NULL	phosphorylated	activate	NULL				enzymes	NULL		SH2 domain		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_28_25323_s_11	12730241	1 Phosphorylated IRSs bind and activate SH2 domain enzymes to couple the  activated receptors to such downstream metabolic effects as glucose uptake and  glycogen and triglyceride synthesis and storage.	bind
16489	3	6171	5	NULL	NULL	0	NULL	statement 1	NULL		occurs simultaneously with	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_28_25323_s_11	12730241	1 Phosphorylated IRSs bind and activate SH2 domain enzymes to couple the  activated receptors to such downstream metabolic effects as glucose uptake and  glycogen and triglyceride synthesis and storage.	bind
16490	4	6171	5	NULL	NULL	0	NULL	statement 3	NULL		leads to	NULL				glucose	NULL	uptake of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_28_25323_s_11	12730241	1 Phosphorylated IRSs bind and activate SH2 domain enzymes to couple the  activated receptors to such downstream metabolic effects as glucose uptake and  glycogen and triglyceride synthesis and storage.	bind
16491	5	6171	5	10	NULL	0	NULL	statement 3			leads to					glycogen		synthesis of;;storage of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_28_25323_s_11	12730241	1 Phosphorylated IRSs bind and activate SH2 domain enzymes to couple the  activated receptors to such downstream metabolic effects as glucose uptake and  glycogen and triglyceride synthesis and storage.	bind
16492	6	6171	5	10	NULL	0	NULL	statement 3			leads to					triglyceride		synthesis of;;storage of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_28_25323_s_11	12730241	1 Phosphorylated IRSs bind and activate SH2 domain enzymes to couple the  activated receptors to such downstream metabolic effects as glucose uptake and  glycogen and triglyceride synthesis and storage.	bind
20842	1	6171	7	NULL	NULL	NULL	NULL	IRSs	GP	phosphorylated	bind					enzymes	GP		SH2 domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_28_25323_s_11	12730241	1 Phosphorylated IRSs bind and activate SH2 domain enzymes to couple the  activated receptors to such downstream metabolic effects as glucose uptake and  glycogen and triglyceride synthesis and storage.	bind
20843	2	6171	7	NULL	NULL	NULL	NULL	IRSs	GP	phosphorylated	activate					enzymes	GP		SH2 domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_28_25323_s_11	12730241	1 Phosphorylated IRSs bind and activate SH2 domain enzymes to couple the  activated receptors to such downstream metabolic effects as glucose uptake and  glycogen and triglyceride synthesis and storage.	bind
20844	3	6171	7	NULL	NULL	NULL	NULL	statement 1	Process		is simultaneous with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_28_25323_s_11	12730241	1 Phosphorylated IRSs bind and activate SH2 domain enzymes to couple the  activated receptors to such downstream metabolic effects as glucose uptake and  glycogen and triglyceride synthesis and storage.	bind
21483	4	6171	7	NULL	NULL	NULL	NULL	statement 3	Process		effect					glucose	Chemical	uptake of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_28_25323_s_11	12730241	1 Phosphorylated IRSs bind and activate SH2 domain enzymes to couple the  activated receptors to such downstream metabolic effects as glucose uptake and  glycogen and triglyceride synthesis and storage.	bind
21484	5	6171	7	NULL	NULL	NULL	NULL	statement 3	Process		effect					glycogen	Chemical	synthesis of;;storage of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_28_25323_s_11	12730241	1 Phosphorylated IRSs bind and activate SH2 domain enzymes to couple the  activated receptors to such downstream metabolic effects as glucose uptake and  glycogen and triglyceride synthesis and storage.	bind
21485	6	6171	7	NULL	NULL	NULL	NULL	statement 3	Process		effect					triglyceride 	Chemical	synthesis of;;storage of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_28_25323_s_11	12730241	1 Phosphorylated IRSs bind and activate SH2 domain enzymes to couple the  activated receptors to such downstream metabolic effects as glucose uptake and  glycogen and triglyceride synthesis and storage.	bind
16494	1	6172	5	10	NULL	0	NULL	E2 envelope glycoprotein	NULL	HCV	bind	NULL				CD81	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_19_19401_s_29	14966136	1 Pileri  et al. ( ) and others ( ,  ,  ) showed that the E2 envelope glycoprotein of HCV binds to CD81.	bind
20849	1	6172	7	NULL	NULL	NULL	NULL	E2 envelope glycoprotein	GP	HCV	binds to					CD81	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_19_19401_s_29	14966136	1 Pileri  et al. ( ) and others ( ,  ,  ) showed that the E2 envelope glycoprotein of HCV binds to CD81.	bind
19285	1	6173	5	NULL	NULL	0	NULL	LHR A	NULL		bind	NULL				iC3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_15_8623_s_143	9535836	1 Recognizes CCP 1  and Enhances iC3 and C4b Binding by LHR A-- Of 20 mAbs to CR1 tested ( 20), 8C9.	bind
19286	2	6173	5	NULL	NULL	0	NULL	LHR A	NULL		bind	NULL				C4b	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_15_8623_s_143	9535836	1 Recognizes CCP 1  and Enhances iC3 and C4b Binding by LHR A-- Of 20 mAbs to CR1 tested ( 20), 8C9.	bind
20850	1	6173	7	NULL	NULL	NULL	NULL	C4b	GP		bind					LHR A	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8623_s_143	9535836	1 Recognizes CCP 1  and Enhances iC3 and C4b Binding by LHR A-- Of 20 mAbs to CR1 tested ( 20), 8C9.	bind
20851	2	6173	7	NULL	NULL	NULL	NULL	 iC3	GP		bind					LHR A	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8623_s_143	9535836	1 Recognizes CCP 1  and Enhances iC3 and C4b Binding by LHR A-- Of 20 mAbs to CR1 tested ( 20), 8C9.	bind
16495	1	6174	5	NULL	NULL	0	NULL	SPIR	NULL		is	NULL				Spironolactone	NULL				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_br-j-pharmacol_148_1_16520746_s_2	16520746	1 Spironolactone (SPIR) binds to cytoplasmic mineralocorticoid receptors  (MR) and functions as an aldosterone antagonist.	bind
16496	2	6174	5	NULL	NULL	0	NULL	MR	NULL		is	NULL				mineralocorticoid receptors	NULL				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_br-j-pharmacol_148_1_16520746_s_2	16520746	1 Spironolactone (SPIR) binds to cytoplasmic mineralocorticoid receptors  (MR) and functions as an aldosterone antagonist.	bind
16497	3	6174	5	NULL	NULL	0	NULL	SPIR	NULL		bind	NULL				MR	NULL	cytoplasmic			NULL		0	NULL	NULL	NULL	abs-batch0700-0719_br-j-pharmacol_148_1_16520746_s_2	16520746	1 Spironolactone (SPIR) binds to cytoplasmic mineralocorticoid receptors  (MR) and functions as an aldosterone antagonist.	bind
16498	4	6174	5	NULL	NULL	0	NULL	SPIR	NULL		function as	NULL				aldosterone antagonist	NULL				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_br-j-pharmacol_148_1_16520746_s_2	16520746	1 Spironolactone (SPIR) binds to cytoplasmic mineralocorticoid receptors  (MR) and functions as an aldosterone antagonist.	bind
20852	1	6174	7	NULL	NULL	NULL	NULL	SPIR	Chemical		binds to					MR	GP	cytoplasmic			NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_br-j-pharmacol_148_1_16520746_s_2	16520746	1 Spironolactone (SPIR) binds to cytoplasmic mineralocorticoid receptors  (MR) and functions as an aldosterone antagonist.	bind
20853	2	6174	7	NULL	NULL	NULL	NULL	SPIR	Chemical		functions as					aldosterone antagonist	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_br-j-pharmacol_148_1_16520746_s_2	16520746	1 Spironolactone (SPIR) binds to cytoplasmic mineralocorticoid receptors  (MR) and functions as an aldosterone antagonist.	bind
20855	3	6174	7	NULL	NULL	NULL	NULL	SPIR	Chemical		is					Spironolactone	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_br-j-pharmacol_148_1_16520746_s_2	16520746	1 Spironolactone (SPIR) binds to cytoplasmic mineralocorticoid receptors  (MR) and functions as an aldosterone antagonist.	bind
20862	4	6174	7	NULL	NULL	NULL	NULL	MR	GP		is					mineralocorticoid receptors	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_br-j-pharmacol_148_1_16520746_s_2	16520746	1 Spironolactone (SPIR) binds to cytoplasmic mineralocorticoid receptors  (MR) and functions as an aldosterone antagonist.	bind
16499	1	6175	5	NULL	NULL	0	NULL	AhR	NULL		is	NULL				aryl hydrocarbon receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_10_6770_s_14	10702233	1 TCDD binds and activates the aryl hydrocarbon receptor (AhR), a member of the basic helix-loop-helix family of transcription factors.	bind
16500	2	6175	5	NULL	NULL	0	NULL	TCDD	NULL		bind	NULL				AhR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_10_6770_s_14	10702233	1 TCDD binds and activates the aryl hydrocarbon receptor (AhR), a member of the basic helix-loop-helix family of transcription factors.	bind
16501	3	6175	5	NULL	NULL	0	NULL	TCDD	NULL		activates	NULL				AhR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_10_6770_s_14	10702233	1 TCDD binds and activates the aryl hydrocarbon receptor (AhR), a member of the basic helix-loop-helix family of transcription factors.	bind
24544	4	6175	5	NULL	NULL	0	NULL	AhR	NULL		is a member of	NULL				basic helix-loop-helix family of transcription factors	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_10_6770_s_14	10702233	1 TCDD binds and activates the aryl hydrocarbon receptor (AhR), a member of the basic helix-loop-helix family of transcription factors.	bind
20865	1	6175	7	NULL	NULL	NULL	NULL	TCDD	Chemical		binds					AhR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_10_6770_s_14	10702233	1 TCDD binds and activates the aryl hydrocarbon receptor (AhR), a member of the basic helix-loop-helix family of transcription factors.	bind
20867	2	6175	7	NULL	NULL	NULL	NULL	TCDD	Chemical		activates					AhR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_10_6770_s_14	10702233	1 TCDD binds and activates the aryl hydrocarbon receptor (AhR), a member of the basic helix-loop-helix family of transcription factors.	bind
20880	3	6175	7	NULL	NULL	NULL	NULL	AhR	GP		member of					basic helix-loop-helix family of transcription factors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_10_6770_s_14	10702233	1 TCDD binds and activates the aryl hydrocarbon receptor (AhR), a member of the basic helix-loop-helix family of transcription factors.	bind
20882	4	6175	7	NULL	NULL	NULL	NULL	AhR	GP		is					aryl hydrocarbon receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_10_6770_s_14	10702233	1 TCDD binds and activates the aryl hydrocarbon receptor (AhR), a member of the basic helix-loop-helix family of transcription factors.	bind
16502	1	6209	5	NULL	NULL	0	NULL	Mint proteins	NULL		bind	NULL	high affinity			Munc18-1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_50_31459_s_140	9395480	1 The following evidence supports the notion that Mint proteins bind to Munc18-1 with high affinity.	bind
20895	1	6209	7	NULL	NULL	NULL	NULL	Mint protein	GP		bind		high affinity			Munc18-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31459_s_140	9395480	1 The following evidence supports the notion that Mint proteins bind to Munc18-1 with high affinity.	bind
16503	1	6210	5	NULL	NULL	0	NULL	CDK inhibitors	NULL		bind	NULL				cyclin-CDK complexes	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_1_175_s_17	9665478	1 The kinase activity of CDKs can be inhibited by a group of CDK inhibitors that bind to cyclin-CDK complexes and block progression through the cell cycle.	bind
16504	2	6210	5	NULL	NULL	0	NULL	statement 1	NULL		block	NULL				cell cycle	NULL	progression through			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_1_175_s_17	9665478	1 The kinase activity of CDKs can be inhibited by a group of CDK inhibitors that bind to cyclin-CDK complexes and block progression through the cell cycle.	bind
16505	3	6210	5	NULL	NULL	0	NULL	CDKs	NULL	kinase activity of	inhibited by	NULL				CDK inhibitors	NULL	group of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_1_175_s_17	9665478	1 The kinase activity of CDKs can be inhibited by a group of CDK inhibitors that bind to cyclin-CDK complexes and block progression through the cell cycle.	bind
20896	1	6210	7	NULL	NULL	NULL	NULL	CDK  inhibitors	Chemical		inhibit					CDKs	GP	kinase activity of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_1_175_s_17	9665478	1 The kinase activity of CDKs can be inhibited by a group of CDK inhibitors that bind to cyclin-CDK complexes and block progression through the cell cycle.	bind
20897	2	6210	7	NULL	NULL	NULL	NULL	CDK inhibitors	Chemical		bind					cyclin-CDK complexes	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_1_175_s_17	9665478	1 The kinase activity of CDKs can be inhibited by a group of CDK inhibitors that bind to cyclin-CDK complexes and block progression through the cell cycle.	bind
20898	3	6210	7	NULL	NULL	NULL	NULL	statement 2	Process		block					cell cycle	Process	progression through			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_1_175_s_17	9665478	1 The kinase activity of CDKs can be inhibited by a group of CDK inhibitors that bind to cyclin-CDK complexes and block progression through the cell cycle.	bind
16506	1	6211	5	NULL	NULL	0	NULL	genomic DNA fragments	NULL	chicken	bind	NULL				v-Myb	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_31_21986_s_29	10419522	1 The Myb consensus sequence was first deduced by isolation of chicken genomic DNA fragments bound by v-Myb on filters ( 13) and from comparison of putative Myb binding sites within the SV40 enhancer ( 14).	bind
20907	1	6211	7	NULL	NULL	NULL	NULL	genomic DNA fragments	NucleicAcid	chicken	bind					v-Myb	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_31_21986_s_29	10419522	1 The Myb consensus sequence was first deduced by isolation of chicken genomic DNA fragments bound by v-Myb on filters ( 13) and from comparison of putative Myb binding sites within the SV40 enhancer ( 14).	bind
16507	1	6212	5	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				BSF lysate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_48_32102_s_192	9822686	1 The pattern of GTP-bound bands was essentially identical, while significantly more GTP was bound by BSF lysate than procyclic.	bind
20917	1	6212	7	NULL	NULL	NULL	NULL	BSF lysate	OrganismPart		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_48_32102_s_192	9822686	1 The pattern of GTP-bound bands was essentially identical, while significantly more GTP was bound by BSF lysate than procyclic.	bind
16575	1	6213	5	NULL	NULL	0	NULL	fibrinogen	NULL		bind	NULL				GP IIb/IIa complex	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_104_12_1374_s_15	11560852	1 The primary mechanism of action of GP IIb/IIIa antagonists is inhibition of the final common pathway of platelet aggregation: fibrinogen or von Willebrand factor binding to the GP IIb/IIa complex.	bind
16576	2	6213	5	NULL	NULL	0	NULL	von Willebrand factor	NULL		bind	NULL				GP IIb/IIa complex	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_104_12_1374_s_15	11560852	1 The primary mechanism of action of GP IIb/IIIa antagonists is inhibition of the final common pathway of platelet aggregation: fibrinogen or von Willebrand factor binding to the GP IIb/IIa complex.	bind
16577	3	6213	5	NULL	NULL	0	NULL	GP IIb/IIIa antagonists	NULL		inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_104_12_1374_s_15	11560852	1 The primary mechanism of action of GP IIb/IIIa antagonists is inhibition of the final common pathway of platelet aggregation: fibrinogen or von Willebrand factor binding to the GP IIb/IIa complex.	bind
16578	4	6213	5	NULL	NULL	0	NULL	GP IIb/IIIa antagonists	NULL		inhibit	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_104_12_1374_s_15	11560852	1 The primary mechanism of action of GP IIb/IIIa antagonists is inhibition of the final common pathway of platelet aggregation: fibrinogen or von Willebrand factor binding to the GP IIb/IIa complex.	bind
20918	1	6213	7	NULL	NULL	NULL	NULL	fibrinogen	GP		bind					GP IIb/IIa complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_12_1374_s_15	11560852	1 The primary mechanism of action of GP IIb/IIIa antagonists is inhibition of the final common pathway of platelet aggregation: fibrinogen or von Willebrand factor binding to the GP IIb/IIa complex.	bind
20919	2	6213	7	NULL	NULL	NULL	NULL	von Willebrand factor	GP		bind					GP IIb/IIa complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_12_1374_s_15	11560852	1 The primary mechanism of action of GP IIb/IIIa antagonists is inhibition of the final common pathway of platelet aggregation: fibrinogen or von Willebrand factor binding to the GP IIb/IIa complex.	bind
20920	3	6213	7	NULL	NULL	NULL	NULL	GP IIb/IIIa antagonists	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_12_1374_s_15	11560852	1 The primary mechanism of action of GP IIb/IIIa antagonists is inhibition of the final common pathway of platelet aggregation: fibrinogen or von Willebrand factor binding to the GP IIb/IIa complex.	bind
20921	4	6213	7	NULL	NULL	NULL	NULL	GP IIb/IIIa antagonists	GP		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_12_1374_s_15	11560852	1 The primary mechanism of action of GP IIb/IIIa antagonists is inhibition of the final common pathway of platelet aggregation: fibrinogen or von Willebrand factor binding to the GP IIb/IIa complex.	bind
16579	1	6214	5	NULL	NULL	0	NULL	A-GLUT1(DTE)	NULL		bind	NULL				pCMB	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1618_1_8_s_404	14643928	1 The residual DTE in the vesicle suspension (approximately 5  M after cytoskeleton-depletion  in the presence of 0.2 mM DTE and washing once with Tris-HCl buffer [ 8) was diluted two-fold upon anion exchange chromatography to obtain A-GLUT1(DTE) and did not affect the binding of A-GLUT1(DTE) to pCMB-Sepharose 4B significantly.	bind
16580	2	6214	5	NULL	NULL	0	NULL	DTE	NULL	residual in the vesicle suspension	did not affect	NULL	significantly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1618_1_8_s_404	14643928	1 The residual DTE in the vesicle suspension (approximately 5  M after cytoskeleton-depletion  in the presence of 0.2 mM DTE and washing once with Tris-HCl buffer [ 8) was diluted two-fold upon anion exchange chromatography to obtain A-GLUT1(DTE) and did not affect the binding of A-GLUT1(DTE) to pCMB-Sepharose 4B significantly.	bind
20922	1	6214	7	NULL	NULL	NULL	NULL	A-GLUT1(DTE)	Chemical		bind					pCMB	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1618_1_8_s_404	14643928	1 The residual DTE in the vesicle suspension (approximately 5  M after cytoskeleton-depletion  in the presence of 0.2 mM DTE and washing once with Tris-HCl buffer [ 8) was diluted two-fold upon anion exchange chromatography to obtain A-GLUT1(DTE) and did not affect the binding of A-GLUT1(DTE) to pCMB-Sepharose 4B significantly.	bind
24175	2	6214	7	NULL	NULL	NULL	NULL	DTE	Chemical	residual in the vesicle suspension	did not affect		significantly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1618_1_8_s_404	14643928	1 The residual DTE in the vesicle suspension (approximately 5  M after cytoskeleton-depletion  in the presence of 0.2 mM DTE and washing once with Tris-HCl buffer [ 8) was diluted two-fold upon anion exchange chromatography to obtain A-GLUT1(DTE) and did not affect the binding of A-GLUT1(DTE) to pCMB-Sepharose 4B significantly.	bind
16581	1	6215	5	NULL	NULL	0	NULL	APC	NULL		is	NULL				activated protein C	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_9_1371_s_19	9743224	1 The zymogen protein C is converted to the active protease, activated protein C (APC), through proteolytic cleavage by thrombin bound to its endothelial membrane receptor thrombomodulin.	bind
16582	2	6215	5	10	NULL	0	NULL	zymogen protein C	NULL		is converted to	NULL				APC	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_9_1371_s_19	9743224	1 The zymogen protein C is converted to the active protease, activated protein C (APC), through proteolytic cleavage by thrombin bound to its endothelial membrane receptor thrombomodulin.	bind
16583	3	6215	5	10	NULL	0	NULL	thrombin	NULL		bind	NULL				thrombomodulin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_9_1371_s_19	9743224	1 The zymogen protein C is converted to the active protease, activated protein C (APC), through proteolytic cleavage by thrombin bound to its endothelial membrane receptor thrombomodulin.	bind
16584	4	6215	5	NULL	NULL	0	NULL	statement 2	NULL		occurs through	NULL				statement 3	NULL	proteolytic cleavage by			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_9_1371_s_19	9743224	1 The zymogen protein C is converted to the active protease, activated protein C (APC), through proteolytic cleavage by thrombin bound to its endothelial membrane receptor thrombomodulin.	bind
45208	5	6215	5	10	NULL	0	NULL	APC	NULL		is a type of	NULL				active protease	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_9_1371_s_19	9743224	1 The zymogen protein C is converted to the active protease, activated protein C (APC), through proteolytic cleavage by thrombin bound to its endothelial membrane receptor thrombomodulin.	bind
45209	6	6215	5	10	NULL	0	NULL	thrombomodulin \t	NULL		is a type of	NULL				endothelial membrane receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_9_1371_s_19	9743224	1 The zymogen protein C is converted to the active protease, activated protein C (APC), through proteolytic cleavage by thrombin bound to its endothelial membrane receptor thrombomodulin.	bind
20925	1	6215	7	NULL	NULL	NULL	NULL	zymogen protein C	GP		converts to					APC	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_9_1371_s_19	9743224	1 The zymogen protein C is converted to the active protease, activated protein C (APC), through proteolytic cleavage by thrombin bound to its endothelial membrane receptor thrombomodulin.	bind
20926	3	6215	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs through					thrombin	GP	proteolytic cleavage by			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_9_1371_s_19	9743224	1 The zymogen protein C is converted to the active protease, activated protein C (APC), through proteolytic cleavage by thrombin bound to its endothelial membrane receptor thrombomodulin.	bind
20927	2	6215	7	NULL	NULL	NULL	NULL	thrombin	GP		bind					thrombomodulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_9_1371_s_19	9743224	1 The zymogen protein C is converted to the active protease, activated protein C (APC), through proteolytic cleavage by thrombin bound to its endothelial membrane receptor thrombomodulin.	bind
20930	4	6215	7	NULL	NULL	NULL	NULL	APC	GP		is					activated protein C	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_9_1371_s_19	9743224	1 The zymogen protein C is converted to the active protease, activated protein C (APC), through proteolytic cleavage by thrombin bound to its endothelial membrane receptor thrombomodulin.	bind
45210	5	6215	7	NULL	NULL	NULL	NULL	APC	GP		is a type of					active protease	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_9_1371_s_19	9743224	1 The zymogen protein C is converted to the active protease, activated protein C (APC), through proteolytic cleavage by thrombin bound to its endothelial membrane receptor thrombomodulin.	bind
54166	6	6215	7	NULL	NULL	NULL	NULL	thrombomodulin	GP		is a type of					endothelial membrane receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_9_1371_s_19	9743224	1 The zymogen protein C is converted to the active protease, activated protein C (APC), through proteolytic cleavage by thrombin bound to its endothelial membrane receptor thrombomodulin.	bind
16585	1	6217	5	10	NULL	0	NULL	Tim44	NULL		bind	NULL				mtHsp70	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_31608_s_30	16027163	1 Tim44 is a peripheral membrane protein that binds both to mtHsp70 and to the translocation channel and thereby recruits the chaperone to the channel.	bind
16586	2	6217	5	10	NULL	0	NULL	Tim44	NULL		bind	NULL				translocation channel	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_31608_s_30	16027163	1 Tim44 is a peripheral membrane protein that binds both to mtHsp70 and to the translocation channel and thereby recruits the chaperone to the channel.	bind
16587	3	6217	5	10	NULL	0	NULL	statement 2			leads to					statement 5					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_31608_s_30	16027163	1 Tim44 is a peripheral membrane protein that binds both to mtHsp70 and to the translocation channel and thereby recruits the chaperone to the channel.	bind
45300	4	6217	5	10	NULL	0	NULL	Tim44	NULL		is a type of	NULL				peripheral membrane protein	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_36_31608_s_30	16027163	1 Tim44 is a peripheral membrane protein that binds both to mtHsp70 and to the translocation channel and thereby recruits the chaperone to the channel.	bind
54167	5	6217	5	10	NULL	0	NULL	chaperone			is recruited to					channel					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_36_31608_s_30	16027163	1 Tim44 is a peripheral membrane protein that binds both to mtHsp70 and to the translocation channel and thereby recruits the chaperone to the channel.	bind
20934	1	6217	7	NULL	NULL	NULL	NULL	Tim44	GP		binds					mtHsp70	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_31608_s_30	16027163	1 Tim44 is a peripheral membrane protein that binds both to mtHsp70 and to the translocation channel and thereby recruits the chaperone to the channel.	bind
20935	2	6217	7	NULL	NULL	NULL	NULL	Tim44	GP		binds					translocation channel	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_31608_s_30	16027163	1 Tim44 is a peripheral membrane protein that binds both to mtHsp70 and to the translocation channel and thereby recruits the chaperone to the channel.	bind
20936	3	6217	7	NULL	NULL	NULL	NULL	statement 2	Process		leads to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_31608_s_30	16027163	1 Tim44 is a peripheral membrane protein that binds both to mtHsp70 and to the translocation channel and thereby recruits the chaperone to the channel.	bind
45301	4	6217	7	NULL	NULL	NULL	NULL	Tim44	GP		is a type of					peripheral membrane protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_31608_s_30	16027163	1 Tim44 is a peripheral membrane protein that binds both to mtHsp70 and to the translocation channel and thereby recruits the chaperone to the channel.	bind
54168	5	6217	7	NULL	NULL	NULL	NULL	chaperone	GP		is recruited to					channel	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_31608_s_30	16027163	1 Tim44 is a peripheral membrane protein that binds both to mtHsp70 and to the translocation channel and thereby recruits the chaperone to the channel.	bind
16588	1	6218	5	NULL	NULL	0	NULL	BPA	NULL		is	NULL				bisphenol A	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_138_7_1271_s_2	12711627	1 We investigated the effect of bisphenol A (BPA), which binds estrogen receptors, on immune responses including production of antigen-specific antibodies, proliferative responses of lymphoid cells, and Th1 and Th2 responses.	bind
16589	2	6218	5	NULL	NULL	0	NULL	BPA	NULL		bind	NULL				estrogen receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_138_7_1271_s_2	12711627	1 We investigated the effect of bisphenol A (BPA), which binds estrogen receptors, on immune responses including production of antigen-specific antibodies, proliferative responses of lymphoid cells, and Th1 and Th2 responses.	bind
20937	1	6218	7	NULL	NULL	NULL	NULL	BPA	Chemical		binds					 estrogen receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_7_1271_s_2	12711627	1 We investigated the effect of bisphenol A (BPA), which binds estrogen receptors, on immune responses including production of antigen-specific antibodies, proliferative responses of lymphoid cells, and Th1 and Th2 responses.	bind
20938	2	6218	7	NULL	NULL	NULL	NULL	BPA	Chemical		is					bisphenol A	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_7_1271_s_2	12711627	1 We investigated the effect of bisphenol A (BPA), which binds estrogen receptors, on immune responses including production of antigen-specific antibodies, proliferative responses of lymphoid cells, and Th1 and Th2 responses.	bind
16590	1	6219	5	NULL	NULL	0	NULL	TF	NULL		bind	NULL				factor VII	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_96_12_4232_s_15	9416887	1 When exposed to blood, TF binds to factor VII, and the resulting complex activates factors IX and X, leading to thrombin and fibrin generation.	bind
16591	2	6219	5	10	NULL	0	NULL	statement 1			occurs on					blood		exposure to			NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_12_4232_s_15	9416887	1 When exposed to blood, TF binds to factor VII, and the resulting complex activates factors IX and X, leading to thrombin and fibrin generation.	bind
16592	3	6219	5	NULL	NULL	0	NULL	statement 1	NULL		activate	NULL				factor IX	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_96_12_4232_s_15	9416887	1 When exposed to blood, TF binds to factor VII, and the resulting complex activates factors IX and X, leading to thrombin and fibrin generation.	bind
16593	4	6219	5	NULL	NULL	0	NULL	statement 1	NULL		activate	NULL				factor X	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_96_12_4232_s_15	9416887	1 When exposed to blood, TF binds to factor VII, and the resulting complex activates factors IX and X, leading to thrombin and fibrin generation.	bind
16594	5	6219	5	NULL	NULL	0	NULL	statement 3	NULL		leads to	NULL				thrombin	NULL	generation of			NULL		0	NULL	NULL	NULL	gw60_circulation_96_12_4232_s_15	9416887	1 When exposed to blood, TF binds to factor VII, and the resulting complex activates factors IX and X, leading to thrombin and fibrin generation.	bind
16595	6	6219	5	NULL	NULL	0	NULL	statement 3	NULL		leads to	NULL				fibrin	NULL	generation of			NULL		0	NULL	NULL	NULL	gw60_circulation_96_12_4232_s_15	9416887	1 When exposed to blood, TF binds to factor VII, and the resulting complex activates factors IX and X, leading to thrombin and fibrin generation.	bind
16596	7	6219	5	NULL	NULL	0	NULL	statement 4	NULL		leads to	NULL				thrombin	NULL	generation of			NULL		0	NULL	NULL	NULL	gw60_circulation_96_12_4232_s_15	9416887	1 When exposed to blood, TF binds to factor VII, and the resulting complex activates factors IX and X, leading to thrombin and fibrin generation.	bind
16597	8	6219	5	NULL	NULL	0	NULL	statement 4	NULL		leads to	NULL				fibrin	NULL	generation of			NULL		0	NULL	NULL	NULL	gw60_circulation_96_12_4232_s_15	9416887	1 When exposed to blood, TF binds to factor VII, and the resulting complex activates factors IX and X, leading to thrombin and fibrin generation.	bind
20939	1	6219	7	NULL	NULL	NULL	NULL	TF	GP		binds to					factor VII	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_12_4232_s_15	9416887	1 When exposed to blood, TF binds to factor VII, and the resulting complex activates factors IX and X, leading to thrombin and fibrin generation.	bind
20940	2	6219	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs upon					blood	OrganismPart	exposure to			NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_12_4232_s_15	9416887	1 When exposed to blood, TF binds to factor VII, and the resulting complex activates factors IX and X, leading to thrombin and fibrin generation.	bind
20941	3	6219	7	NULL	NULL	NULL	NULL	statement 1	Process		activates					factors IX	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_12_4232_s_15	9416887	1 When exposed to blood, TF binds to factor VII, and the resulting complex activates factors IX and X, leading to thrombin and fibrin generation.	bind
20942	4	6219	7	NULL	NULL	NULL	NULL	statement 1	Process		activates					factor X	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_12_4232_s_15	9416887	1 When exposed to blood, TF binds to factor VII, and the resulting complex activates factors IX and X, leading to thrombin and fibrin generation.	bind
20943	5	6219	7	NULL	NULL	NULL	NULL	statement 3	Process		leads to					thrombin	GP	generation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_12_4232_s_15	9416887	1 When exposed to blood, TF binds to factor VII, and the resulting complex activates factors IX and X, leading to thrombin and fibrin generation.	bind
20944	6	6219	7	NULL	NULL	NULL	NULL	statement 3	Process		leads to					fibrin	GP	generation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_12_4232_s_15	9416887	1 When exposed to blood, TF binds to factor VII, and the resulting complex activates factors IX and X, leading to thrombin and fibrin generation.	bind
20945	7	6219	7	NULL	NULL	NULL	NULL	statement 4	Process		leads to					thrombin	GP	generation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_12_4232_s_15	9416887	1 When exposed to blood, TF binds to factor VII, and the resulting complex activates factors IX and X, leading to thrombin and fibrin generation.	bind
20946	8	6219	7	NULL	NULL	NULL	NULL	statement 4	Process		leads to					fibrin	GP	generation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_12_4232_s_15	9416887	1 When exposed to blood, TF binds to factor VII, and the resulting complex activates factors IX and X, leading to thrombin and fibrin generation.	bind
16600	1	6220	5	NULL	NULL	0	NULL	GST CD-MPR peptide	NULL		bind	NULL					NULL		VHS domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_21_18477_s_118	11886874	1% of the pellet ( P) and supernatant ( S) were resolved on 10% SDS gels, transferred to nitrocellulose, and probed with either the anti-Myc or anti-HA antibody as described under   *, highlights the fact that the GST CD-MPR peptide does bind to the VHS domain albeit very weakly relative to the GST CI-MPR peptide, 25% of pellet and 5% of supernatant were loaded in this case.	bind
16604	2	6220	5	NULL	NULL	0	NULL	GST CI-MPR peptide	NULL		bind	NULL					NULL		VHS domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_21_18477_s_118	11886874	1% of the pellet ( P) and supernatant ( S) were resolved on 10% SDS gels, transferred to nitrocellulose, and probed with either the anti-Myc or anti-HA antibody as described under   *, highlights the fact that the GST CD-MPR peptide does bind to the VHS domain albeit very weakly relative to the GST CI-MPR peptide, 25% of pellet and 5% of supernatant were loaded in this case.	bind
16605	3	6220	5	NULL	NULL	0	NULL	statement 1	NULL		very weak relative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_21_18477_s_118	11886874	1% of the pellet ( P) and supernatant ( S) were resolved on 10% SDS gels, transferred to nitrocellulose, and probed with either the anti-Myc or anti-HA antibody as described under   *, highlights the fact that the GST CD-MPR peptide does bind to the VHS domain albeit very weakly relative to the GST CI-MPR peptide, 25% of pellet and 5% of supernatant were loaded in this case.	bind
21007	1	6220	7	NULL	NULL	NULL	NULL	GST CD-MPR peptide	GP		bind		weakly						VHS domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_21_18477_s_118	11886874	1% of the pellet ( P) and supernatant ( S) were resolved on 10% SDS gels, transferred to nitrocellulose, and probed with either the anti-Myc or anti-HA antibody as described under   *, highlights the fact that the GST CD-MPR peptide does bind to the VHS domain albeit very weakly relative to the GST CI-MPR peptide, 25% of pellet and 5% of supernatant were loaded in this case.	bind
21008	2	6220	7	NULL	NULL	NULL	NULL	GST CI-MPR peptide	GP		bind								VHS domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_21_18477_s_118	11886874	1% of the pellet ( P) and supernatant ( S) were resolved on 10% SDS gels, transferred to nitrocellulose, and probed with either the anti-Myc or anti-HA antibody as described under   *, highlights the fact that the GST CD-MPR peptide does bind to the VHS domain albeit very weakly relative to the GST CI-MPR peptide, 25% of pellet and 5% of supernatant were loaded in this case.	bind
21009	3	6220	7	NULL	NULL	NULL	NULL	statement 1	Process		is weaker than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_21_18477_s_118	11886874	1% of the pellet ( P) and supernatant ( S) were resolved on 10% SDS gels, transferred to nitrocellulose, and probed with either the anti-Myc or anti-HA antibody as described under   *, highlights the fact that the GST CD-MPR peptide does bind to the VHS domain albeit very weakly relative to the GST CI-MPR peptide, 25% of pellet and 5% of supernatant were loaded in this case.	bind
16610	1	6221	5	10	NULL	0	NULL	FXI	NULL	bound	is associated with	NULL				membrane rafts	NULL				NULL	TRAP-activated platelets	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_24_21744_s_192	12517745	1)   5 - 8% of bound FXI is associated with membrane rafts in  TRAP-activated platelets (Figs.   2 and   3,  A and  B);  2) FXI-raft association was disrupted by cholesterol depletion  ( Fig. 4); 3) FXI binds to lipid  rafts through the A3 domain ( Fig.  6 A); 4) the SZ-2 antibody blocks the binding of FXI to  lipid rafts suggesting FXI interacts with GPIb in lipid rafts  ( Fig. 6 B); and 5) the  initial rate of FXI activation by thrombin on activated platelets was  inhibited >85% by cholesterol depletion leading to raft disruption  ( Fig. 7).	bind
16612	2	6221	5	10	NULL	0	NULL	cholesterol	NULL	depletion of	disrupt	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_24_21744_s_192	12517745	1)   5 - 8% of bound FXI is associated with membrane rafts in  TRAP-activated platelets (Figs.   2 and   3,  A and  B);  2) FXI-raft association was disrupted by cholesterol depletion  ( Fig. 4); 3) FXI binds to lipid  rafts through the A3 domain ( Fig.  6 A); 4) the SZ-2 antibody blocks the binding of FXI to  lipid rafts suggesting FXI interacts with GPIb in lipid rafts  ( Fig. 6 B); and 5) the  initial rate of FXI activation by thrombin on activated platelets was  inhibited >85% by cholesterol depletion leading to raft disruption  ( Fig. 7).	bind
16613	3	6221	5	NULL	NULL	0	NULL	FXI	NULL		bind	NULL		A3 domain		lipid rafts	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_24_21744_s_192	12517745	1)   5 - 8% of bound FXI is associated with membrane rafts in  TRAP-activated platelets (Figs.   2 and   3,  A and  B);  2) FXI-raft association was disrupted by cholesterol depletion  ( Fig. 4); 3) FXI binds to lipid  rafts through the A3 domain ( Fig.  6 A); 4) the SZ-2 antibody blocks the binding of FXI to  lipid rafts suggesting FXI interacts with GPIb in lipid rafts  ( Fig. 6 B); and 5) the  initial rate of FXI activation by thrombin on activated platelets was  inhibited >85% by cholesterol depletion leading to raft disruption  ( Fig. 7).	bind
16615	4	6221	5	NULL	NULL	0	NULL	SZ-2 antibody	NULL		block	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_24_21744_s_192	12517745	1)   5 - 8% of bound FXI is associated with membrane rafts in  TRAP-activated platelets (Figs.   2 and   3,  A and  B);  2) FXI-raft association was disrupted by cholesterol depletion  ( Fig. 4); 3) FXI binds to lipid  rafts through the A3 domain ( Fig.  6 A); 4) the SZ-2 antibody blocks the binding of FXI to  lipid rafts suggesting FXI interacts with GPIb in lipid rafts  ( Fig. 6 B); and 5) the  initial rate of FXI activation by thrombin on activated platelets was  inhibited >85% by cholesterol depletion leading to raft disruption  ( Fig. 7).	bind
16616	5	6221	5	NULL	NULL	0	NULL	FXI	NULL		interact with	NULL				GPIb	NULL				NULL	in lipid rafts	0	NULL	NULL	NULL	gw70_jbiolchem_278_24_21744_s_192	12517745	1)   5 - 8% of bound FXI is associated with membrane rafts in  TRAP-activated platelets (Figs.   2 and   3,  A and  B);  2) FXI-raft association was disrupted by cholesterol depletion  ( Fig. 4); 3) FXI binds to lipid  rafts through the A3 domain ( Fig.  6 A); 4) the SZ-2 antibody blocks the binding of FXI to  lipid rafts suggesting FXI interacts with GPIb in lipid rafts  ( Fig. 6 B); and 5) the  initial rate of FXI activation by thrombin on activated platelets was  inhibited >85% by cholesterol depletion leading to raft disruption  ( Fig. 7).	bind
16618	6	6221	5	NULL	NULL	0	NULL	statement 4	NULL		suggest	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_24_21744_s_192	12517745	1)   5 - 8% of bound FXI is associated with membrane rafts in  TRAP-activated platelets (Figs.   2 and   3,  A and  B);  2) FXI-raft association was disrupted by cholesterol depletion  ( Fig. 4); 3) FXI binds to lipid  rafts through the A3 domain ( Fig.  6 A); 4) the SZ-2 antibody blocks the binding of FXI to  lipid rafts suggesting FXI interacts with GPIb in lipid rafts  ( Fig. 6 B); and 5) the  initial rate of FXI activation by thrombin on activated platelets was  inhibited >85% by cholesterol depletion leading to raft disruption  ( Fig. 7).	bind
16622	7	6221	5	NULL	NULL	0	NULL	thrombin	NULL		activate	NULL				FXI	NULL				NULL	on activated platelets	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_24_21744_s_192	12517745	1)   5 - 8% of bound FXI is associated with membrane rafts in  TRAP-activated platelets (Figs.   2 and   3,  A and  B);  2) FXI-raft association was disrupted by cholesterol depletion  ( Fig. 4); 3) FXI binds to lipid  rafts through the A3 domain ( Fig.  6 A); 4) the SZ-2 antibody blocks the binding of FXI to  lipid rafts suggesting FXI interacts with GPIb in lipid rafts  ( Fig. 6 B); and 5) the  initial rate of FXI activation by thrombin on activated platelets was  inhibited >85% by cholesterol depletion leading to raft disruption  ( Fig. 7).	bind
16625	8	6221	5	10	NULL	0	NULL	cholesterol	NULL	depletion of 	inhibit	NULL				statement 7	NULL	initial rate of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_24_21744_s_192	12517745	1)   5 - 8% of bound FXI is associated with membrane rafts in  TRAP-activated platelets (Figs.   2 and   3,  A and  B);  2) FXI-raft association was disrupted by cholesterol depletion  ( Fig. 4); 3) FXI binds to lipid  rafts through the A3 domain ( Fig.  6 A); 4) the SZ-2 antibody blocks the binding of FXI to  lipid rafts suggesting FXI interacts with GPIb in lipid rafts  ( Fig. 6 B); and 5) the  initial rate of FXI activation by thrombin on activated platelets was  inhibited >85% by cholesterol depletion leading to raft disruption  ( Fig. 7).	bind
16627	9	6221	5	10	NULL	0	NULL	statement 8			leads to					raft		disruption of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_24_21744_s_192	12517745	1)   5 - 8% of bound FXI is associated with membrane rafts in  TRAP-activated platelets (Figs.   2 and   3,  A and  B);  2) FXI-raft association was disrupted by cholesterol depletion  ( Fig. 4); 3) FXI binds to lipid  rafts through the A3 domain ( Fig.  6 A); 4) the SZ-2 antibody blocks the binding of FXI to  lipid rafts suggesting FXI interacts with GPIb in lipid rafts  ( Fig. 6 B); and 5) the  initial rate of FXI activation by thrombin on activated platelets was  inhibited >85% by cholesterol depletion leading to raft disruption  ( Fig. 7).	bind
21010	1	6221	7	NULL	NULL	NULL	NULL	FXI	GP	bound	associate with					membrane rafts	CellComponent				NULL	TRAP-activated platelets	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_24_21744_s_192	12517745	1)   5 - 8% of bound FXI is associated with membrane rafts in  TRAP-activated platelets (Figs.   2 and   3,  A and  B);  2) FXI-raft association was disrupted by cholesterol depletion  ( Fig. 4); 3) FXI binds to lipid  rafts through the A3 domain ( Fig.  6 A); 4) the SZ-2 antibody blocks the binding of FXI to  lipid rafts suggesting FXI interacts with GPIb in lipid rafts  ( Fig. 6 B); and 5) the  initial rate of FXI activation by thrombin on activated platelets was  inhibited >85% by cholesterol depletion leading to raft disruption  ( Fig. 7).	bind
21011	2	6221	7	NULL	NULL	NULL	NULL	cholesterol	Chemical	depletion of	disrupts					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_24_21744_s_192	12517745	1)   5 - 8% of bound FXI is associated with membrane rafts in  TRAP-activated platelets (Figs.   2 and   3,  A and  B);  2) FXI-raft association was disrupted by cholesterol depletion  ( Fig. 4); 3) FXI binds to lipid  rafts through the A3 domain ( Fig.  6 A); 4) the SZ-2 antibody blocks the binding of FXI to  lipid rafts suggesting FXI interacts with GPIb in lipid rafts  ( Fig. 6 B); and 5) the  initial rate of FXI activation by thrombin on activated platelets was  inhibited >85% by cholesterol depletion leading to raft disruption  ( Fig. 7).	bind
21012	3	6221	7	NULL	NULL	NULL	NULL	FXI 	GP		bind			A3 domain		lipid rafts	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_24_21744_s_192	12517745	1)   5 - 8% of bound FXI is associated with membrane rafts in  TRAP-activated platelets (Figs.   2 and   3,  A and  B);  2) FXI-raft association was disrupted by cholesterol depletion  ( Fig. 4); 3) FXI binds to lipid  rafts through the A3 domain ( Fig.  6 A); 4) the SZ-2 antibody blocks the binding of FXI to  lipid rafts suggesting FXI interacts with GPIb in lipid rafts  ( Fig. 6 B); and 5) the  initial rate of FXI activation by thrombin on activated platelets was  inhibited >85% by cholesterol depletion leading to raft disruption  ( Fig. 7).	bind
21013	4	6221	7	NULL	NULL	NULL	NULL	 SZ-2 antibody	GP		blocks					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_24_21744_s_192	12517745	1)   5 - 8% of bound FXI is associated with membrane rafts in  TRAP-activated platelets (Figs.   2 and   3,  A and  B);  2) FXI-raft association was disrupted by cholesterol depletion  ( Fig. 4); 3) FXI binds to lipid  rafts through the A3 domain ( Fig.  6 A); 4) the SZ-2 antibody blocks the binding of FXI to  lipid rafts suggesting FXI interacts with GPIb in lipid rafts  ( Fig. 6 B); and 5) the  initial rate of FXI activation by thrombin on activated platelets was  inhibited >85% by cholesterol depletion leading to raft disruption  ( Fig. 7).	bind
21014	5	6221	7	NULL	NULL	NULL	NULL	FXI	GP		interacts with					GPIb	GP				NULL	lipid rafts	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_24_21744_s_192	12517745	1)   5 - 8% of bound FXI is associated with membrane rafts in  TRAP-activated platelets (Figs.   2 and   3,  A and  B);  2) FXI-raft association was disrupted by cholesterol depletion  ( Fig. 4); 3) FXI binds to lipid  rafts through the A3 domain ( Fig.  6 A); 4) the SZ-2 antibody blocks the binding of FXI to  lipid rafts suggesting FXI interacts with GPIb in lipid rafts  ( Fig. 6 B); and 5) the  initial rate of FXI activation by thrombin on activated platelets was  inhibited >85% by cholesterol depletion leading to raft disruption  ( Fig. 7).	bind
21015	6	6221	7	NULL	NULL	NULL	NULL	thrombin	GP		activates					FXI	GP				NULL	activated platelets	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_24_21744_s_192	12517745	1)   5 - 8% of bound FXI is associated with membrane rafts in  TRAP-activated platelets (Figs.   2 and   3,  A and  B);  2) FXI-raft association was disrupted by cholesterol depletion  ( Fig. 4); 3) FXI binds to lipid  rafts through the A3 domain ( Fig.  6 A); 4) the SZ-2 antibody blocks the binding of FXI to  lipid rafts suggesting FXI interacts with GPIb in lipid rafts  ( Fig. 6 B); and 5) the  initial rate of FXI activation by thrombin on activated platelets was  inhibited >85% by cholesterol depletion leading to raft disruption  ( Fig. 7).	bind
21016	7	6221	7	NULL	NULL	NULL	NULL	cholesterol	Chemical	depletion of	inhibits					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_24_21744_s_192	12517745	1)   5 - 8% of bound FXI is associated with membrane rafts in  TRAP-activated platelets (Figs.   2 and   3,  A and  B);  2) FXI-raft association was disrupted by cholesterol depletion  ( Fig. 4); 3) FXI binds to lipid  rafts through the A3 domain ( Fig.  6 A); 4) the SZ-2 antibody blocks the binding of FXI to  lipid rafts suggesting FXI interacts with GPIb in lipid rafts  ( Fig. 6 B); and 5) the  initial rate of FXI activation by thrombin on activated platelets was  inhibited >85% by cholesterol depletion leading to raft disruption  ( Fig. 7).	bind
21017	8	6221	7	NULL	NULL	NULL	NULL	statement 7	Process		disrupts					rafts	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_24_21744_s_192	12517745	1)   5 - 8% of bound FXI is associated with membrane rafts in  TRAP-activated platelets (Figs.   2 and   3,  A and  B);  2) FXI-raft association was disrupted by cholesterol depletion  ( Fig. 4); 3) FXI binds to lipid  rafts through the A3 domain ( Fig.  6 A); 4) the SZ-2 antibody blocks the binding of FXI to  lipid rafts suggesting FXI interacts with GPIb in lipid rafts  ( Fig. 6 B); and 5) the  initial rate of FXI activation by thrombin on activated platelets was  inhibited >85% by cholesterol depletion leading to raft disruption  ( Fig. 7).	bind
19280	1	6222	5	NULL	NULL	0	NULL	ADIP	NULL		bind	NULL				alpha-actinin	NULL				NULL	extracts of HEK293 cells exogenously expressing full-length ADIP	NULL	NULL	NULL	NULL	gw60_jbiolchem_278_6_4103_s_301	12446711	1) ADIP binds to alpha-actinin as estimated by the yeast two-hybrid analysis and co-immunoprecipitation from the extracts of HEK293 cells exogenously expressing the full-length ADIP or fragments; 2) recombinant ADIP directly binds to recombinant alpha-actinin in a cell-free system; and 3) endogenous ADIP and alpha-actinin are co-immunoprecipitated from the extracts of MDCK cells.	bind
19281	2	6222	5	NULL	NULL	0	NULL	ADIP	NULL		bind	NULL				alpha-actinin	NULL				NULL	extracts of HEK293 cells exogenously expressing fragments of ADIP	0	NULL	NULL	NULL	gw60_jbiolchem_278_6_4103_s_301	12446711	1) ADIP binds to alpha-actinin as estimated by the yeast two-hybrid analysis and co-immunoprecipitation from the extracts of HEK293 cells exogenously expressing the full-length ADIP or fragments; 2) recombinant ADIP directly binds to recombinant alpha-actinin in a cell-free system; and 3) endogenous ADIP and alpha-actinin are co-immunoprecipitated from the extracts of MDCK cells.	bind
19282	3	6222	5	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_6_4103_s_301	12446711	1) ADIP binds to alpha-actinin as estimated by the yeast two-hybrid analysis and co-immunoprecipitation from the extracts of HEK293 cells exogenously expressing the full-length ADIP or fragments; 2) recombinant ADIP directly binds to recombinant alpha-actinin in a cell-free system; and 3) endogenous ADIP and alpha-actinin are co-immunoprecipitated from the extracts of MDCK cells.	bind
19283	4	6222	5	NULL	NULL	0	NULL	ADIP	NULL	recombinant	bind	NULL	directly			alpha-actinin	NULL	recombinant			NULL	cell-free system	0	NULL	NULL	NULL	gw60_jbiolchem_278_6_4103_s_301	12446711	1) ADIP binds to alpha-actinin as estimated by the yeast two-hybrid analysis and co-immunoprecipitation from the extracts of HEK293 cells exogenously expressing the full-length ADIP or fragments; 2) recombinant ADIP directly binds to recombinant alpha-actinin in a cell-free system; and 3) endogenous ADIP and alpha-actinin are co-immunoprecipitated from the extracts of MDCK cells.	bind
19284	5	6222	5	NULL	NULL	0	NULL	ADIP	NULL	endogenous	bind	NULL				alpha-actinin	NULL	endogenous			NULL	extracts of MDCK cells	0	NULL	NULL	NULL	gw60_jbiolchem_278_6_4103_s_301	12446711	1) ADIP binds to alpha-actinin as estimated by the yeast two-hybrid analysis and co-immunoprecipitation from the extracts of HEK293 cells exogenously expressing the full-length ADIP or fragments; 2) recombinant ADIP directly binds to recombinant alpha-actinin in a cell-free system; and 3) endogenous ADIP and alpha-actinin are co-immunoprecipitated from the extracts of MDCK cells.	bind
21018	1	6222	7	NULL	NULL	NULL	NULL	 ADIP	GP		bind					alpha-actinin	GP				NULL	HEK293 cells exogenously expressing the full-length ADIP	NULL	NULL	NULL	NULL	gw60_jbiolchem_278_6_4103_s_301	12446711	1) ADIP binds to alpha-actinin as estimated by the yeast two-hybrid analysis and co-immunoprecipitation from the extracts of HEK293 cells exogenously expressing the full-length ADIP or fragments; 2) recombinant ADIP directly binds to recombinant alpha-actinin in a cell-free system; and 3) endogenous ADIP and alpha-actinin are co-immunoprecipitated from the extracts of MDCK cells.	bind
21019	2	6222	7	NULL	NULL	NULL	NULL	ADIP	GP		bind					alpha-actinin	GP				NULL	HEK293 cells exogenously expressing the ADIP fragments	NULL	NULL	NULL	NULL	gw60_jbiolchem_278_6_4103_s_301	12446711	1) ADIP binds to alpha-actinin as estimated by the yeast two-hybrid analysis and co-immunoprecipitation from the extracts of HEK293 cells exogenously expressing the full-length ADIP or fragments; 2) recombinant ADIP directly binds to recombinant alpha-actinin in a cell-free system; and 3) endogenous ADIP and alpha-actinin are co-immunoprecipitated from the extracts of MDCK cells.	bind
21020	3	6222	7	NULL	NULL	NULL	NULL	ADIP	GP	recombinant	bind		directly			alpha-actinin	GP	recombinant			NULL	in a cell-free system	NULL	NULL	NULL	NULL	gw60_jbiolchem_278_6_4103_s_301	12446711	1) ADIP binds to alpha-actinin as estimated by the yeast two-hybrid analysis and co-immunoprecipitation from the extracts of HEK293 cells exogenously expressing the full-length ADIP or fragments; 2) recombinant ADIP directly binds to recombinant alpha-actinin in a cell-free system; and 3) endogenous ADIP and alpha-actinin are co-immunoprecipitated from the extracts of MDCK cells.	bind
21021	4	6222	7	NULL	NULL	NULL	NULL	ADIP 	GP	endogenous	bind					alpha-actinin	GP				NULL	MDCK cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_278_6_4103_s_301	12446711	1) ADIP binds to alpha-actinin as estimated by the yeast two-hybrid analysis and co-immunoprecipitation from the extracts of HEK293 cells exogenously expressing the full-length ADIP or fragments; 2) recombinant ADIP directly binds to recombinant alpha-actinin in a cell-free system; and 3) endogenous ADIP and alpha-actinin are co-immunoprecipitated from the extracts of MDCK cells.	bind
55020	5	6222	7	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_6_4103_s_301	12446711	1) ADIP binds to alpha-actinin as estimated by the yeast two-hybrid analysis and co-immunoprecipitation from the extracts of HEK293 cells exogenously expressing the full-length ADIP or fragments; 2) recombinant ADIP directly binds to recombinant alpha-actinin in a cell-free system; and 3) endogenous ADIP and alpha-actinin are co-immunoprecipitated from the extracts of MDCK cells.	bind
16629	1	6223	5	NULL	NULL	0	NULL	Agmatine	NULL		displace	NULL				MK-801	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_288_2_544_s_150	9918557	1) Agmatine is 10- to 100-fold more potent in displacing MK-801 binding than putrescine or spermine, respectively (Anis et al., 1990  ).	bind
16630	2	6223	5	NULL	NULL	0	NULL	putrescine	NULL		displace	NULL				MK-801	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_288_2_544_s_150	9918557	1) Agmatine is 10- to 100-fold more potent in displacing MK-801 binding than putrescine or spermine, respectively (Anis et al., 1990  ).	bind
16632	3	6223	5	NULL	NULL	0	NULL	spermine	NULL		displace	NULL				MK-801	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_288_2_544_s_150	9918557	1) Agmatine is 10- to 100-fold more potent in displacing MK-801 binding than putrescine or spermine, respectively (Anis et al., 1990  ).	bind
16634	4	6223	5	NULL	NULL	0	NULL	statement 1	NULL		more potent than	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_288_2_544_s_150	9918557	1) Agmatine is 10- to 100-fold more potent in displacing MK-801 binding than putrescine or spermine, respectively (Anis et al., 1990  ).	bind
16636	5	6223	5	NULL	NULL	0	NULL	statement 1	NULL		more potent than	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_288_2_544_s_150	9918557	1) Agmatine is 10- to 100-fold more potent in displacing MK-801 binding than putrescine or spermine, respectively (Anis et al., 1990  ).	bind
21022	1	6223	7	NULL	NULL	NULL	NULL	Agmatine	Chemical		displace		significantly			MK-801	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_288_2_544_s_150	9918557	1) Agmatine is 10- to 100-fold more potent in displacing MK-801 binding than putrescine or spermine, respectively (Anis et al., 1990  ).	bind
21023	2	6223	7	NULL	NULL	NULL	NULL	putrescine	Chemical		displace					MK-801	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_288_2_544_s_150	9918557	1) Agmatine is 10- to 100-fold more potent in displacing MK-801 binding than putrescine or spermine, respectively (Anis et al., 1990  ).	bind
21024	3	6223	7	NULL	NULL	NULL	NULL	spermine	Chemical		displace					MK-801	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_288_2_544_s_150	9918557	1) Agmatine is 10- to 100-fold more potent in displacing MK-801 binding than putrescine or spermine, respectively (Anis et al., 1990  ).	bind
21025	4	6223	7	NULL	NULL	NULL	NULL	statement 1	Process		is more potent than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_288_2_544_s_150	9918557	1) Agmatine is 10- to 100-fold more potent in displacing MK-801 binding than putrescine or spermine, respectively (Anis et al., 1990  ).	bind
21026	5	6223	7	NULL	NULL	NULL	NULL	statement 1	Process		is more potent than					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_288_2_544_s_150	9918557	1) Agmatine is 10- to 100-fold more potent in displacing MK-801 binding than putrescine or spermine, respectively (Anis et al., 1990  ).	bind
16642	1	6224	5	NULL	NULL	0	NULL	one G protein trimer 	NULL	only	bind	NULL				B4 receptor BLT1 dimeric complex	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24108_s_259	15056658	1) Applying chemical cross-linking of purified leukotriene B4 receptor BLT1 and Galphai2, beta1, and gamma2 proteins in a reconstituted system, Baneres and Parello ( ) used a combination of mass spectrometry and neutron scattering to established that only one G protein trimer binds to the dimeric complex of this receptor.	bind
21486	1	6224	7	NULL	NULL	NULL	NULL	G protein trimer	GP		binds					 BLT1 dimeric complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_23_24108_s_259	15056658	1) Applying chemical cross-linking of purified leukotriene B4 receptor BLT1 and Galphai2, beta1, and gamma2 proteins in a reconstituted system, Baneres and Parello ( ) used a combination of mass spectrometry and neutron scattering to established that only one G protein trimer binds to the dimeric complex of this receptor.	bind
67931	2	6224	7	NULL	NULL	0	NULL	BLT1	GP		is a type of					leukotriene B4 receptor	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24108_s_259	15056658	1) Applying chemical cross-linking of purified leukotriene B4 receptor BLT1 and Galphai2, beta1, and gamma2 proteins in a reconstituted system, Baneres and Parello ( ) used a combination of mass spectrometry and neutron scattering to established that only one G protein trimer binds to the dimeric complex of this receptor.	bind
16647	1	6225	5	NULL	NULL	0	NULL	N-end rule pathway	NULL		degrade	NULL				Arg-e -DHFRha	NULL				NULL	in ATP-supplemented reticulocyte extract	0	NULL	NULL	NULL	gw60_jbiolchem_270_14_8172_s_143	7713922	1) Arg-e -DHFRha ( Fig. 1 ) is degraded by the N-end  rule pathway in ATP-supplemented reticulocyte extract in the absence  but not in the presence of MTX, a folic acid analog and a competitive  inhibitor of DHFR which binds to mammalian DHFRs with a  K   of  10 M  ( Fig. 3  A).	bind
16648	2	6225	5	NULL	NULL	0	NULL	statement 1	NULL		in the absence of	NULL				MTX	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_14_8172_s_143	7713922	1) Arg-e -DHFRha ( Fig. 1 ) is degraded by the N-end  rule pathway in ATP-supplemented reticulocyte extract in the absence  but not in the presence of MTX, a folic acid analog and a competitive  inhibitor of DHFR which binds to mammalian DHFRs with a  K   of  10 M  ( Fig. 3  A).	bind
16649	3	6225	5	NULL	NULL	0	NULL	MTX	NULL		is a type of	NULL				folic acid analog	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_14_8172_s_143	7713922	1) Arg-e -DHFRha ( Fig. 1 ) is degraded by the N-end  rule pathway in ATP-supplemented reticulocyte extract in the absence  but not in the presence of MTX, a folic acid analog and a competitive  inhibitor of DHFR which binds to mammalian DHFRs with a  K   of  10 M  ( Fig. 3  A).	bind
16650	4	6225	5	NULL	NULL	0	NULL	MTX	NULL		is a type of	NULL				DHFR inhibitor	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_14_8172_s_143	7713922	1) Arg-e -DHFRha ( Fig. 1 ) is degraded by the N-end  rule pathway in ATP-supplemented reticulocyte extract in the absence  but not in the presence of MTX, a folic acid analog and a competitive  inhibitor of DHFR which binds to mammalian DHFRs with a  K   of  10 M  ( Fig. 3  A).	bind
16651	5	6225	5	NULL	NULL	0	NULL	MTX	NULL		bind	NULL				DHFR	NULL	mammalian			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_14_8172_s_143	7713922	1) Arg-e -DHFRha ( Fig. 1 ) is degraded by the N-end  rule pathway in ATP-supplemented reticulocyte extract in the absence  but not in the presence of MTX, a folic acid analog and a competitive  inhibitor of DHFR which binds to mammalian DHFRs with a  K   of  10 M  ( Fig. 3  A).	bind
21066	1	6225	7	NULL	NULL	NULL	NULL	 Arg-e -DHFRha 	GP		is degraded by					N-end rule pathway	Process				NULL	ATP-supplemented reticulocyte extract	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_14_8172_s_143	7713922	1) Arg-e -DHFRha ( Fig. 1 ) is degraded by the N-end  rule pathway in ATP-supplemented reticulocyte extract in the absence  but not in the presence of MTX, a folic acid analog and a competitive  inhibitor of DHFR which binds to mammalian DHFRs with a  K   of  10 M  ( Fig. 3  A).	bind
21067	2	6225	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs in the absence of					MTX	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_14_8172_s_143	7713922	1) Arg-e -DHFRha ( Fig. 1 ) is degraded by the N-end  rule pathway in ATP-supplemented reticulocyte extract in the absence  but not in the presence of MTX, a folic acid analog and a competitive  inhibitor of DHFR which binds to mammalian DHFRs with a  K   of  10 M  ( Fig. 3  A).	bind
21068	3	6225	7	NULL	NULL	NULL	NULL	statement 1	Process		does not occur					MTX	Chemical	in the presence of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_14_8172_s_143	7713922	1) Arg-e -DHFRha ( Fig. 1 ) is degraded by the N-end  rule pathway in ATP-supplemented reticulocyte extract in the absence  but not in the presence of MTX, a folic acid analog and a competitive  inhibitor of DHFR which binds to mammalian DHFRs with a  K   of  10 M  ( Fig. 3  A).	bind
21069	4	6225	7	NULL	NULL	NULL	NULL	MTX	Chemical		is a type of					folic acid analog	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_14_8172_s_143	7713922	1) Arg-e -DHFRha ( Fig. 1 ) is degraded by the N-end  rule pathway in ATP-supplemented reticulocyte extract in the absence  but not in the presence of MTX, a folic acid analog and a competitive  inhibitor of DHFR which binds to mammalian DHFRs with a  K   of  10 M  ( Fig. 3  A).	bind
21070	5	6225	7	NULL	NULL	NULL	NULL	MTX	Chemical		is a type of					DHFR inhibitor	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_14_8172_s_143	7713922	1) Arg-e -DHFRha ( Fig. 1 ) is degraded by the N-end  rule pathway in ATP-supplemented reticulocyte extract in the absence  but not in the presence of MTX, a folic acid analog and a competitive  inhibitor of DHFR which binds to mammalian DHFRs with a  K   of  10 M  ( Fig. 3  A).	bind
26351	6	6225	7	NULL	NULL	NULL	NULL	MTX	Chemical		bind					DHFR	GP	mammalian			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_14_8172_s_143	7713922	1) Arg-e -DHFRha ( Fig. 1 ) is degraded by the N-end  rule pathway in ATP-supplemented reticulocyte extract in the absence  but not in the presence of MTX, a folic acid analog and a competitive  inhibitor of DHFR which binds to mammalian DHFRs with a  K   of  10 M  ( Fig. 3  A).	bind
16652	1	6226	5	NULL	NULL	0	NULL	ArgBP2	NULL		is localized in	NULL				stress fibers	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_28_17542_s_250	9211900	1) ArgBP2, like cytoplasmic c-Abl, is localized in stress fibers; 2) ArgBP2 directly associates with Arg and v-Abl in living cells; 3) ArgBP2 is a substrate for Abl family kinases, consistent with the observation that it has several sequences that conform to the suggested peptide target for the Abl kinase; 4) endogenous ArgBP2 is phosphorylated on tyrosine residues in NIH3T3 cells transformed by v-Abl, a dysregulated Abl oncoprotein; and 5) the mechanism of ArgBP2 binding with Abl family kinases is specific (the first and third ArgBP2 SH3 domains interact with the second of three proline-rich motifs located in the Arg and c-Abl COOH-terminal domains).	bind
16653	2	6226	5	NULL	NULL	0	NULL	c-Abl	NULL	cytoplasmic	is localized in	NULL				stress fibers	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_28_17542_s_250	9211900	1) ArgBP2, like cytoplasmic c-Abl, is localized in stress fibers; 2) ArgBP2 directly associates with Arg and v-Abl in living cells; 3) ArgBP2 is a substrate for Abl family kinases, consistent with the observation that it has several sequences that conform to the suggested peptide target for the Abl kinase; 4) endogenous ArgBP2 is phosphorylated on tyrosine residues in NIH3T3 cells transformed by v-Abl, a dysregulated Abl oncoprotein; and 5) the mechanism of ArgBP2 binding with Abl family kinases is specific (the first and third ArgBP2 SH3 domains interact with the second of three proline-rich motifs located in the Arg and c-Abl COOH-terminal domains).	bind
16654	3	6226	5	NULL	NULL	0	NULL	ArgBP2	NULL		associate with	NULL	directly			Arg	NULL				NULL	in living cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17542_s_250	9211900	1) ArgBP2, like cytoplasmic c-Abl, is localized in stress fibers; 2) ArgBP2 directly associates with Arg and v-Abl in living cells; 3) ArgBP2 is a substrate for Abl family kinases, consistent with the observation that it has several sequences that conform to the suggested peptide target for the Abl kinase; 4) endogenous ArgBP2 is phosphorylated on tyrosine residues in NIH3T3 cells transformed by v-Abl, a dysregulated Abl oncoprotein; and 5) the mechanism of ArgBP2 binding with Abl family kinases is specific (the first and third ArgBP2 SH3 domains interact with the second of three proline-rich motifs located in the Arg and c-Abl COOH-terminal domains).	bind
16655	4	6226	5	NULL	NULL	0	NULL	ArgBP2	NULL		associate with	NULL	directly			v-Abl	NULL				NULL	in living cells	0	NULL	NULL	NULL	gw60_jbiolchem_272_28_17542_s_250	9211900	1) ArgBP2, like cytoplasmic c-Abl, is localized in stress fibers; 2) ArgBP2 directly associates with Arg and v-Abl in living cells; 3) ArgBP2 is a substrate for Abl family kinases, consistent with the observation that it has several sequences that conform to the suggested peptide target for the Abl kinase; 4) endogenous ArgBP2 is phosphorylated on tyrosine residues in NIH3T3 cells transformed by v-Abl, a dysregulated Abl oncoprotein; and 5) the mechanism of ArgBP2 binding with Abl family kinases is specific (the first and third ArgBP2 SH3 domains interact with the second of three proline-rich motifs located in the Arg and c-Abl COOH-terminal domains).	bind
16656	5	6226	5	NULL	NULL	0	NULL	ArgBP2	NULL		is a substrate for	NULL				Abl family kinases	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_28_17542_s_250	9211900	1) ArgBP2, like cytoplasmic c-Abl, is localized in stress fibers; 2) ArgBP2 directly associates with Arg and v-Abl in living cells; 3) ArgBP2 is a substrate for Abl family kinases, consistent with the observation that it has several sequences that conform to the suggested peptide target for the Abl kinase; 4) endogenous ArgBP2 is phosphorylated on tyrosine residues in NIH3T3 cells transformed by v-Abl, a dysregulated Abl oncoprotein; and 5) the mechanism of ArgBP2 binding with Abl family kinases is specific (the first and third ArgBP2 SH3 domains interact with the second of three proline-rich motifs located in the Arg and c-Abl COOH-terminal domains).	bind
16657	6	6226	5	NULL	NULL	0	NULL	ArgBP2	NULL	endogenous	undergoes	NULL		tyrosine residues		phosphorylation	NULL				NULL	in NIH3T3 cells transformed by v-Abl, a dysregulated Abl oncoprotein	0	NULL	NULL	NULL	gw60_jbiolchem_272_28_17542_s_250	9211900	1) ArgBP2, like cytoplasmic c-Abl, is localized in stress fibers; 2) ArgBP2 directly associates with Arg and v-Abl in living cells; 3) ArgBP2 is a substrate for Abl family kinases, consistent with the observation that it has several sequences that conform to the suggested peptide target for the Abl kinase; 4) endogenous ArgBP2 is phosphorylated on tyrosine residues in NIH3T3 cells transformed by v-Abl, a dysregulated Abl oncoprotein; and 5) the mechanism of ArgBP2 binding with Abl family kinases is specific (the first and third ArgBP2 SH3 domains interact with the second of three proline-rich motifs located in the Arg and c-Abl COOH-terminal domains).	bind
16658	7	6226	5	NULL	NULL	0	NULL	ArgBP2	NULL		bind	NULL	specific			Abl family kinases	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_28_17542_s_250	9211900	1) ArgBP2, like cytoplasmic c-Abl, is localized in stress fibers; 2) ArgBP2 directly associates with Arg and v-Abl in living cells; 3) ArgBP2 is a substrate for Abl family kinases, consistent with the observation that it has several sequences that conform to the suggested peptide target for the Abl kinase; 4) endogenous ArgBP2 is phosphorylated on tyrosine residues in NIH3T3 cells transformed by v-Abl, a dysregulated Abl oncoprotein; and 5) the mechanism of ArgBP2 binding with Abl family kinases is specific (the first and third ArgBP2 SH3 domains interact with the second of three proline-rich motifs located in the Arg and c-Abl COOH-terminal domains).	bind
16659	8	6226	5	NULL	NULL	0	NULL	ArgBP2	NULL		interact with	NULL		first SH3 domain		Arg	NULL		second of three proline-rich motifs		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17542_s_250	9211900	1) ArgBP2, like cytoplasmic c-Abl, is localized in stress fibers; 2) ArgBP2 directly associates with Arg and v-Abl in living cells; 3) ArgBP2 is a substrate for Abl family kinases, consistent with the observation that it has several sequences that conform to the suggested peptide target for the Abl kinase; 4) endogenous ArgBP2 is phosphorylated on tyrosine residues in NIH3T3 cells transformed by v-Abl, a dysregulated Abl oncoprotein; and 5) the mechanism of ArgBP2 binding with Abl family kinases is specific (the first and third ArgBP2 SH3 domains interact with the second of three proline-rich motifs located in the Arg and c-Abl COOH-terminal domains).	bind
16660	9	6226	5	NULL	NULL	0	NULL	ArgBP2	NULL		interact with	NULL		third SH3 domain		Arg	NULL		second of three proline-rich motifs		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_28_17542_s_250	9211900	1) ArgBP2, like cytoplasmic c-Abl, is localized in stress fibers; 2) ArgBP2 directly associates with Arg and v-Abl in living cells; 3) ArgBP2 is a substrate for Abl family kinases, consistent with the observation that it has several sequences that conform to the suggested peptide target for the Abl kinase; 4) endogenous ArgBP2 is phosphorylated on tyrosine residues in NIH3T3 cells transformed by v-Abl, a dysregulated Abl oncoprotein; and 5) the mechanism of ArgBP2 binding with Abl family kinases is specific (the first and third ArgBP2 SH3 domains interact with the second of three proline-rich motifs located in the Arg and c-Abl COOH-terminal domains).	bind
16661	10	6226	5	NULL	NULL	0	NULL	ArgBP2	NULL		interact with	NULL		first SH3 domain		c-Abl	NULL		COOH-terminal domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17542_s_250	9211900	1) ArgBP2, like cytoplasmic c-Abl, is localized in stress fibers; 2) ArgBP2 directly associates with Arg and v-Abl in living cells; 3) ArgBP2 is a substrate for Abl family kinases, consistent with the observation that it has several sequences that conform to the suggested peptide target for the Abl kinase; 4) endogenous ArgBP2 is phosphorylated on tyrosine residues in NIH3T3 cells transformed by v-Abl, a dysregulated Abl oncoprotein; and 5) the mechanism of ArgBP2 binding with Abl family kinases is specific (the first and third ArgBP2 SH3 domains interact with the second of three proline-rich motifs located in the Arg and c-Abl COOH-terminal domains).	bind
16662	11	6226	5	NULL	NULL	0	NULL	ArgBP2	NULL		interact with	NULL		third SH3 domain		c-Abl	NULL		COOH-terminal domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_28_17542_s_250	9211900	1) ArgBP2, like cytoplasmic c-Abl, is localized in stress fibers; 2) ArgBP2 directly associates with Arg and v-Abl in living cells; 3) ArgBP2 is a substrate for Abl family kinases, consistent with the observation that it has several sequences that conform to the suggested peptide target for the Abl kinase; 4) endogenous ArgBP2 is phosphorylated on tyrosine residues in NIH3T3 cells transformed by v-Abl, a dysregulated Abl oncoprotein; and 5) the mechanism of ArgBP2 binding with Abl family kinases is specific (the first and third ArgBP2 SH3 domains interact with the second of three proline-rich motifs located in the Arg and c-Abl COOH-terminal domains).	bind
21071	1	6226	7	NULL	NULL	NULL	NULL	ArgBP2	GP		is localized in					stress fibers	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17542_s_250	9211900	1) ArgBP2, like cytoplasmic c-Abl, is localized in stress fibers; 2) ArgBP2 directly associates with Arg and v-Abl in living cells; 3) ArgBP2 is a substrate for Abl family kinases, consistent with the observation that it has several sequences that conform to the suggested peptide target for the Abl kinase; 4) endogenous ArgBP2 is phosphorylated on tyrosine residues in NIH3T3 cells transformed by v-Abl, a dysregulated Abl oncoprotein; and 5) the mechanism of ArgBP2 binding with Abl family kinases is specific (the first and third ArgBP2 SH3 domains interact with the second of three proline-rich motifs located in the Arg and c-Abl COOH-terminal domains).	bind
21072	2	6226	7	NULL	NULL	NULL	NULL	c-Abl	GP	cytoplasmic	is localized in					stress fibers	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17542_s_250	9211900	1) ArgBP2, like cytoplasmic c-Abl, is localized in stress fibers; 2) ArgBP2 directly associates with Arg and v-Abl in living cells; 3) ArgBP2 is a substrate for Abl family kinases, consistent with the observation that it has several sequences that conform to the suggested peptide target for the Abl kinase; 4) endogenous ArgBP2 is phosphorylated on tyrosine residues in NIH3T3 cells transformed by v-Abl, a dysregulated Abl oncoprotein; and 5) the mechanism of ArgBP2 binding with Abl family kinases is specific (the first and third ArgBP2 SH3 domains interact with the second of three proline-rich motifs located in the Arg and c-Abl COOH-terminal domains).	bind
21073	3	6226	7	NULL	NULL	NULL	NULL	ArgBP2	GP		associate with		directly			Arg 	AminoAcid				NULL	living cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17542_s_250	9211900	1) ArgBP2, like cytoplasmic c-Abl, is localized in stress fibers; 2) ArgBP2 directly associates with Arg and v-Abl in living cells; 3) ArgBP2 is a substrate for Abl family kinases, consistent with the observation that it has several sequences that conform to the suggested peptide target for the Abl kinase; 4) endogenous ArgBP2 is phosphorylated on tyrosine residues in NIH3T3 cells transformed by v-Abl, a dysregulated Abl oncoprotein; and 5) the mechanism of ArgBP2 binding with Abl family kinases is specific (the first and third ArgBP2 SH3 domains interact with the second of three proline-rich motifs located in the Arg and c-Abl COOH-terminal domains).	bind
21074	4	6226	7	NULL	NULL	NULL	NULL	ArgBP2	GP		associate with		directly			v-Abl	GP				NULL	living cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17542_s_250	9211900	1) ArgBP2, like cytoplasmic c-Abl, is localized in stress fibers; 2) ArgBP2 directly associates with Arg and v-Abl in living cells; 3) ArgBP2 is a substrate for Abl family kinases, consistent with the observation that it has several sequences that conform to the suggested peptide target for the Abl kinase; 4) endogenous ArgBP2 is phosphorylated on tyrosine residues in NIH3T3 cells transformed by v-Abl, a dysregulated Abl oncoprotein; and 5) the mechanism of ArgBP2 binding with Abl family kinases is specific (the first and third ArgBP2 SH3 domains interact with the second of three proline-rich motifs located in the Arg and c-Abl COOH-terminal domains).	bind
21075	5	6226	7	NULL	NULL	NULL	NULL	ArgBP2	GP		is a substrate for					Abl family kinases	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17542_s_250	9211900	1) ArgBP2, like cytoplasmic c-Abl, is localized in stress fibers; 2) ArgBP2 directly associates with Arg and v-Abl in living cells; 3) ArgBP2 is a substrate for Abl family kinases, consistent with the observation that it has several sequences that conform to the suggested peptide target for the Abl kinase; 4) endogenous ArgBP2 is phosphorylated on tyrosine residues in NIH3T3 cells transformed by v-Abl, a dysregulated Abl oncoprotein; and 5) the mechanism of ArgBP2 binding with Abl family kinases is specific (the first and third ArgBP2 SH3 domains interact with the second of three proline-rich motifs located in the Arg and c-Abl COOH-terminal domains).	bind
21076	6	6226	7	NULL	NULL	NULL	NULL	ArgBP2	GP	endogenous	is phosphorylated on								tyrosine residues		NULL	NIH3T3 cells transformed by v-Abl	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17542_s_250	9211900	1) ArgBP2, like cytoplasmic c-Abl, is localized in stress fibers; 2) ArgBP2 directly associates with Arg and v-Abl in living cells; 3) ArgBP2 is a substrate for Abl family kinases, consistent with the observation that it has several sequences that conform to the suggested peptide target for the Abl kinase; 4) endogenous ArgBP2 is phosphorylated on tyrosine residues in NIH3T3 cells transformed by v-Abl, a dysregulated Abl oncoprotein; and 5) the mechanism of ArgBP2 binding with Abl family kinases is specific (the first and third ArgBP2 SH3 domains interact with the second of three proline-rich motifs located in the Arg and c-Abl COOH-terminal domains).	bind
21077	7	6226	7	NULL	NULL	NULL	NULL	v-Abl	GP		is					Abl oncoprotein	GP	dysregulated 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17542_s_250	9211900	1) ArgBP2, like cytoplasmic c-Abl, is localized in stress fibers; 2) ArgBP2 directly associates with Arg and v-Abl in living cells; 3) ArgBP2 is a substrate for Abl family kinases, consistent with the observation that it has several sequences that conform to the suggested peptide target for the Abl kinase; 4) endogenous ArgBP2 is phosphorylated on tyrosine residues in NIH3T3 cells transformed by v-Abl, a dysregulated Abl oncoprotein; and 5) the mechanism of ArgBP2 binding with Abl family kinases is specific (the first and third ArgBP2 SH3 domains interact with the second of three proline-rich motifs located in the Arg and c-Abl COOH-terminal domains).	bind
21078	8	6226	7	NULL	NULL	NULL	NULL	ArgBP2	GP		bind		specifically			Abl family kinases	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17542_s_250	9211900	1) ArgBP2, like cytoplasmic c-Abl, is localized in stress fibers; 2) ArgBP2 directly associates with Arg and v-Abl in living cells; 3) ArgBP2 is a substrate for Abl family kinases, consistent with the observation that it has several sequences that conform to the suggested peptide target for the Abl kinase; 4) endogenous ArgBP2 is phosphorylated on tyrosine residues in NIH3T3 cells transformed by v-Abl, a dysregulated Abl oncoprotein; and 5) the mechanism of ArgBP2 binding with Abl family kinases is specific (the first and third ArgBP2 SH3 domains interact with the second of three proline-rich motifs located in the Arg and c-Abl COOH-terminal domains).	bind
21080	9	6226	7	NULL	NULL	NULL	NULL	ArgBP2	GP		interact with			first SH3 domain		c-Abl	GP		second proline-rich motifs located in the Arg domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17542_s_250	9211900	1) ArgBP2, like cytoplasmic c-Abl, is localized in stress fibers; 2) ArgBP2 directly associates with Arg and v-Abl in living cells; 3) ArgBP2 is a substrate for Abl family kinases, consistent with the observation that it has several sequences that conform to the suggested peptide target for the Abl kinase; 4) endogenous ArgBP2 is phosphorylated on tyrosine residues in NIH3T3 cells transformed by v-Abl, a dysregulated Abl oncoprotein; and 5) the mechanism of ArgBP2 binding with Abl family kinases is specific (the first and third ArgBP2 SH3 domains interact with the second of three proline-rich motifs located in the Arg and c-Abl COOH-terminal domains).	bind
21081	10	6226	7	NULL	NULL	NULL	NULL	ArgBP2	GP		interact with			first SH3 domain		c-Abl	GP		second proline-rich motifs located in the COOH-terminal domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17542_s_250	9211900	1) ArgBP2, like cytoplasmic c-Abl, is localized in stress fibers; 2) ArgBP2 directly associates with Arg and v-Abl in living cells; 3) ArgBP2 is a substrate for Abl family kinases, consistent with the observation that it has several sequences that conform to the suggested peptide target for the Abl kinase; 4) endogenous ArgBP2 is phosphorylated on tyrosine residues in NIH3T3 cells transformed by v-Abl, a dysregulated Abl oncoprotein; and 5) the mechanism of ArgBP2 binding with Abl family kinases is specific (the first and third ArgBP2 SH3 domains interact with the second of three proline-rich motifs located in the Arg and c-Abl COOH-terminal domains).	bind
55028	11	6226	7	NULL	NULL	NULL	NULL	ArgBP2	GP		interact with			third SH3 domain		c-Abl	GP		second of three proline-rich motifs located in the Arg domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17542_s_250	9211900	1) ArgBP2, like cytoplasmic c-Abl, is localized in stress fibers; 2) ArgBP2 directly associates with Arg and v-Abl in living cells; 3) ArgBP2 is a substrate for Abl family kinases, consistent with the observation that it has several sequences that conform to the suggested peptide target for the Abl kinase; 4) endogenous ArgBP2 is phosphorylated on tyrosine residues in NIH3T3 cells transformed by v-Abl, a dysregulated Abl oncoprotein; and 5) the mechanism of ArgBP2 binding with Abl family kinases is specific (the first and third ArgBP2 SH3 domains interact with the second of three proline-rich motifs located in the Arg and c-Abl COOH-terminal domains).	bind
55029	12	6226	7	NULL	NULL	NULL	NULL	ArgBP2	GP		interact with			third SH3 domain		c-Abl	GP		COOH-terminal domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17542_s_250	9211900	1) ArgBP2, like cytoplasmic c-Abl, is localized in stress fibers; 2) ArgBP2 directly associates with Arg and v-Abl in living cells; 3) ArgBP2 is a substrate for Abl family kinases, consistent with the observation that it has several sequences that conform to the suggested peptide target for the Abl kinase; 4) endogenous ArgBP2 is phosphorylated on tyrosine residues in NIH3T3 cells transformed by v-Abl, a dysregulated Abl oncoprotein; and 5) the mechanism of ArgBP2 binding with Abl family kinases is specific (the first and third ArgBP2 SH3 domains interact with the second of three proline-rich motifs located in the Arg and c-Abl COOH-terminal domains).	bind
16663	1	6227	5	NULL	NULL	0	NULL	NtpK	NULL	ion binding site	bind	NULL	high affinity	Glu-139		Na+	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_27_24405_s_162	11983695	1) At the first step of ion translocation, the ion binding site on NtpK (Glu-139) binds Na+ with a single high affinity ( Kd of Na+ = 15  plus-or-minus  5 muM) ( 15).	bind
16664	2	6227	5	NULL	NULL	0	NULL	statement 1	NULL		occurs at	NULL				first step of ion translocation	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_27_24405_s_162	11983695	1) At the first step of ion translocation, the ion binding site on NtpK (Glu-139) binds Na+ with a single high affinity ( Kd of Na+ = 15  plus-or-minus  5 muM) ( 15).	bind
21082	1	6227	7	NULL	NULL	NULL	NULL	 NtpK	GP		bind		high affinity	Glu-139		Na+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_27_24405_s_162	11983695	1) At the first step of ion translocation, the ion binding site on NtpK (Glu-139) binds Na+ with a single high affinity ( Kd of Na+ = 15  plus-or-minus  5 muM) ( 15).	bind
26352	2	6227	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs at					first step of ion translocation	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_27_24405_s_162	11983695	1) At the first step of ion translocation, the ion binding site on NtpK (Glu-139) binds Na+ with a single high affinity ( Kd of Na+ = 15  plus-or-minus  5 muM) ( 15).	bind
16665	1	6228	5	NULL	NULL	0	NULL	Bernard-Soulier platelets	NULL		is deficient in	NULL				factor XI	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_3_1662_s_4	11696542	1) Bernard-Soulier platelets, lacking the complex, are deficient in factor XI binding; 2) two GP Ibalpha ligands, SZ-2 (a monoclonal antibody) and bovine von Willebrand factor, inhibit factor XI binding to platelets; 3) by surface plasmon resonance, factor XI bound specifically to glycocalicin (the extracellular domain of GP Ibalpha) in Zn2+-dependent fashion ( K d app ~ 52 nM).	bind
16666	2	6228	5	NULL	NULL	0	NULL	factor XI	NULL		bind	NULL				platelets	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_3_1662_s_4	11696542	1) Bernard-Soulier platelets, lacking the complex, are deficient in factor XI binding; 2) two GP Ibalpha ligands, SZ-2 (a monoclonal antibody) and bovine von Willebrand factor, inhibit factor XI binding to platelets; 3) by surface plasmon resonance, factor XI bound specifically to glycocalicin (the extracellular domain of GP Ibalpha) in Zn2+-dependent fashion ( K d app ~ 52 nM).	bind
16667	3	6228	5	NULL	NULL	0	NULL	two GP Ibalpha ligands	NULL		inhibit	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_3_1662_s_4	11696542	1) Bernard-Soulier platelets, lacking the complex, are deficient in factor XI binding; 2) two GP Ibalpha ligands, SZ-2 (a monoclonal antibody) and bovine von Willebrand factor, inhibit factor XI binding to platelets; 3) by surface plasmon resonance, factor XI bound specifically to glycocalicin (the extracellular domain of GP Ibalpha) in Zn2+-dependent fashion ( K d app ~ 52 nM).	bind
16668	4	6228	5	NULL	NULL	0	NULL	SZ-2	NULL		inhibit	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_3_1662_s_4	11696542	1) Bernard-Soulier platelets, lacking the complex, are deficient in factor XI binding; 2) two GP Ibalpha ligands, SZ-2 (a monoclonal antibody) and bovine von Willebrand factor, inhibit factor XI binding to platelets; 3) by surface plasmon resonance, factor XI bound specifically to glycocalicin (the extracellular domain of GP Ibalpha) in Zn2+-dependent fashion ( K d app ~ 52 nM).	bind
16669	5	6228	5	10	NULL	0	NULL	SZ-2			is a type of					monoclonal antibody					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_1662_s_4	11696542	1) Bernard-Soulier platelets, lacking the complex, are deficient in factor XI binding; 2) two GP Ibalpha ligands, SZ-2 (a monoclonal antibody) and bovine von Willebrand factor, inhibit factor XI binding to platelets; 3) by surface plasmon resonance, factor XI bound specifically to glycocalicin (the extracellular domain of GP Ibalpha) in Zn2+-dependent fashion ( K d app ~ 52 nM).	bind
16670	6	6228	5	NULL	NULL	0	NULL	von Willebrand factor	NULL	bovine	inhibit	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_3_1662_s_4	11696542	1) Bernard-Soulier platelets, lacking the complex, are deficient in factor XI binding; 2) two GP Ibalpha ligands, SZ-2 (a monoclonal antibody) and bovine von Willebrand factor, inhibit factor XI binding to platelets; 3) by surface plasmon resonance, factor XI bound specifically to glycocalicin (the extracellular domain of GP Ibalpha) in Zn2+-dependent fashion ( K d app ~ 52 nM).	bind
16671	7	6228	5	NULL	NULL	0	NULL	factor XI	NULL		bind	NULL	specifically			glycocalicin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_3_1662_s_4	11696542	1) Bernard-Soulier platelets, lacking the complex, are deficient in factor XI binding; 2) two GP Ibalpha ligands, SZ-2 (a monoclonal antibody) and bovine von Willebrand factor, inhibit factor XI binding to platelets; 3) by surface plasmon resonance, factor XI bound specifically to glycocalicin (the extracellular domain of GP Ibalpha) in Zn2+-dependent fashion ( K d app ~ 52 nM).	bind
16672	8	6228	5	NULL	NULL	0	NULL	glycocalicin	NULL		is	NULL				extracellular domain of GP Ibalpha	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_3_1662_s_4	11696542	1) Bernard-Soulier platelets, lacking the complex, are deficient in factor XI binding; 2) two GP Ibalpha ligands, SZ-2 (a monoclonal antibody) and bovine von Willebrand factor, inhibit factor XI binding to platelets; 3) by surface plasmon resonance, factor XI bound specifically to glycocalicin (the extracellular domain of GP Ibalpha) in Zn2+-dependent fashion ( K d app ~ 52 nM).	bind
16673	9	6228	5	NULL	NULL	0	NULL	statement 7	NULL		dependent on	NULL				Zn2+	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_3_1662_s_4	11696542	1) Bernard-Soulier platelets, lacking the complex, are deficient in factor XI binding; 2) two GP Ibalpha ligands, SZ-2 (a monoclonal antibody) and bovine von Willebrand factor, inhibit factor XI binding to platelets; 3) by surface plasmon resonance, factor XI bound specifically to glycocalicin (the extracellular domain of GP Ibalpha) in Zn2+-dependent fashion ( K d app ~ 52 nM).	bind
21083	1	6228	7	NULL	NULL	NULL	NULL	factor XI	GP		bind					platelets	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_1662_s_4	11696542	1) Bernard-Soulier platelets, lacking the complex, are deficient in factor XI binding; 2) two GP Ibalpha ligands, SZ-2 (a monoclonal antibody) and bovine von Willebrand factor, inhibit factor XI binding to platelets; 3) by surface plasmon resonance, factor XI bound specifically to glycocalicin (the extracellular domain of GP Ibalpha) in Zn2+-dependent fashion ( K d app ~ 52 nM).	bind
21084	2	6228	7	NULL	NULL	NULL	NULL	GP Ibalpha ligands	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_1662_s_4	11696542	1) Bernard-Soulier platelets, lacking the complex, are deficient in factor XI binding; 2) two GP Ibalpha ligands, SZ-2 (a monoclonal antibody) and bovine von Willebrand factor, inhibit factor XI binding to platelets; 3) by surface plasmon resonance, factor XI bound specifically to glycocalicin (the extracellular domain of GP Ibalpha) in Zn2+-dependent fashion ( K d app ~ 52 nM).	bind
21085	3	6228	7	NULL	NULL	NULL	NULL	SZ-2	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_1662_s_4	11696542	1) Bernard-Soulier platelets, lacking the complex, are deficient in factor XI binding; 2) two GP Ibalpha ligands, SZ-2 (a monoclonal antibody) and bovine von Willebrand factor, inhibit factor XI binding to platelets; 3) by surface plasmon resonance, factor XI bound specifically to glycocalicin (the extracellular domain of GP Ibalpha) in Zn2+-dependent fashion ( K d app ~ 52 nM).	bind
21086	4	6228	7	NULL	NULL	NULL	NULL	 von Willebrand factor	GP	bovine	inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_1662_s_4	11696542	1) Bernard-Soulier platelets, lacking the complex, are deficient in factor XI binding; 2) two GP Ibalpha ligands, SZ-2 (a monoclonal antibody) and bovine von Willebrand factor, inhibit factor XI binding to platelets; 3) by surface plasmon resonance, factor XI bound specifically to glycocalicin (the extracellular domain of GP Ibalpha) in Zn2+-dependent fashion ( K d app ~ 52 nM).	bind
21087	5	6228	7	NULL	NULL	NULL	NULL	factor XI	GP		bind		specifically			glycocalicin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_1662_s_4	11696542	1) Bernard-Soulier platelets, lacking the complex, are deficient in factor XI binding; 2) two GP Ibalpha ligands, SZ-2 (a monoclonal antibody) and bovine von Willebrand factor, inhibit factor XI binding to platelets; 3) by surface plasmon resonance, factor XI bound specifically to glycocalicin (the extracellular domain of GP Ibalpha) in Zn2+-dependent fashion ( K d app ~ 52 nM).	bind
21088	6	6228	7	NULL	NULL	NULL	NULL	statement 5	Process		is dependent on					Zn2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_1662_s_4	11696542	1) Bernard-Soulier platelets, lacking the complex, are deficient in factor XI binding; 2) two GP Ibalpha ligands, SZ-2 (a monoclonal antibody) and bovine von Willebrand factor, inhibit factor XI binding to platelets; 3) by surface plasmon resonance, factor XI bound specifically to glycocalicin (the extracellular domain of GP Ibalpha) in Zn2+-dependent fashion ( K d app ~ 52 nM).	bind
54169	7	6228	7	NULL	NULL	NULL	NULL	SZ-2	GP		is a type of					monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_1662_s_4	11696542	1) Bernard-Soulier platelets, lacking the complex, are deficient in factor XI binding; 2) two GP Ibalpha ligands, SZ-2 (a monoclonal antibody) and bovine von Willebrand factor, inhibit factor XI binding to platelets; 3) by surface plasmon resonance, factor XI bound specifically to glycocalicin (the extracellular domain of GP Ibalpha) in Zn2+-dependent fashion ( K d app ~ 52 nM).	bind
54170	8	6228	7	NULL	NULL	NULL	NULL	Bernard-Soulier platelets	OrganismPart		is deficient in					factor XI	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_1662_s_4	11696542	1) Bernard-Soulier platelets, lacking the complex, are deficient in factor XI binding; 2) two GP Ibalpha ligands, SZ-2 (a monoclonal antibody) and bovine von Willebrand factor, inhibit factor XI binding to platelets; 3) by surface plasmon resonance, factor XI bound specifically to glycocalicin (the extracellular domain of GP Ibalpha) in Zn2+-dependent fashion ( K d app ~ 52 nM).	bind
16674	1	6229	5	NULL	NULL	0	NULL	Wnt protein	NULL		bind	NULL				Frizzled transmembrane receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_2_325_s_17	10027390	1) Binding of the Wnt protein to the Frizzled transmembrane receptor activates the Disheveled protein, which, in turn, inhibits the activity of glycogen synthase kinase 3beta (GSK3beta).	bind
16675	2	6229	5	NULL	NULL	0	NULL	statement 1	NULL		activate	NULL				Disheveled protein	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_2_325_s_17	10027390	1) Binding of the Wnt protein to the Frizzled transmembrane receptor activates the Disheveled protein, which, in turn, inhibits the activity of glycogen synthase kinase 3beta (GSK3beta).	bind
16676	3	6229	5	NULL	NULL	0	NULL	statement 2	NULL		inhibit	NULL				GSK3beta	NULL	activity of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_2_325_s_17	10027390	1) Binding of the Wnt protein to the Frizzled transmembrane receptor activates the Disheveled protein, which, in turn, inhibits the activity of glycogen synthase kinase 3beta (GSK3beta).	bind
16677	4	6229	5	NULL	NULL	0	NULL	GSK3beta	NULL		is	NULL				glycogen synthase kinase 3beta	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_2_325_s_17	10027390	1) Binding of the Wnt protein to the Frizzled transmembrane receptor activates the Disheveled protein, which, in turn, inhibits the activity of glycogen synthase kinase 3beta (GSK3beta).	bind
21089	1	6229	7	NULL	NULL	NULL	NULL	Wnt protein	GP		bind					Frizzled transmembrane receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_2_325_s_17	10027390	1) Binding of the Wnt protein to the Frizzled transmembrane receptor activates the Disheveled protein, which, in turn, inhibits the activity of glycogen synthase kinase 3beta (GSK3beta).	bind
21090	2	6229	7	NULL	NULL	NULL	NULL	statement 1	Process		activates					Disheveled protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_2_325_s_17	10027390	1) Binding of the Wnt protein to the Frizzled transmembrane receptor activates the Disheveled protein, which, in turn, inhibits the activity of glycogen synthase kinase 3beta (GSK3beta).	bind
21091	3	6229	7	NULL	NULL	NULL	NULL	statement 2	Process		inhibits					GSK3beta	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_2_325_s_17	10027390	1) Binding of the Wnt protein to the Frizzled transmembrane receptor activates the Disheveled protein, which, in turn, inhibits the activity of glycogen synthase kinase 3beta (GSK3beta).	bind
21092	4	6229	7	NULL	NULL	NULL	NULL	GSK3beta	GP		is					glycogen synthase kinase 3beta	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_2_325_s_17	10027390	1) Binding of the Wnt protein to the Frizzled transmembrane receptor activates the Disheveled protein, which, in turn, inhibits the activity of glycogen synthase kinase 3beta (GSK3beta).	bind
16678	1	6230	5	NULL	NULL	0	NULL	BMS-345541	NULL		bind	NULL				IKK-1	NULL		ATP binding site		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_3_1450_s_234	12403772	1) BMS-345541 binds to the ATP binding site of IKK-1 but not of IKK-2, or 2) BMS-345541 binds to similar allosteric sites on IKK-1 and IKK-2, but binding to the allosteric site on IKK-2 leads to a conformational change in the enzyme that alters the peptide binding site whereas the conformational change that occurs upon binding of BMS-345541 to the corresponding site on IKK-1 causes a perturbation of the ATP binding site.	bind
16679	2	6230	5	NULL	NULL	0	NULL	BMS-345541	NULL		does not bind	NULL				IKK-2	NULL		ATP binding site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_3_1450_s_234	12403772	1) BMS-345541 binds to the ATP binding site of IKK-1 but not of IKK-2, or 2) BMS-345541 binds to similar allosteric sites on IKK-1 and IKK-2, but binding to the allosteric site on IKK-2 leads to a conformational change in the enzyme that alters the peptide binding site whereas the conformational change that occurs upon binding of BMS-345541 to the corresponding site on IKK-1 causes a perturbation of the ATP binding site.	bind
16680	3	6230	5	NULL	NULL	0	NULL	BMS-345541	NULL		bind	NULL				IKK-1	NULL		similar allosteric sites		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_3_1450_s_234	12403772	1) BMS-345541 binds to the ATP binding site of IKK-1 but not of IKK-2, or 2) BMS-345541 binds to similar allosteric sites on IKK-1 and IKK-2, but binding to the allosteric site on IKK-2 leads to a conformational change in the enzyme that alters the peptide binding site whereas the conformational change that occurs upon binding of BMS-345541 to the corresponding site on IKK-1 causes a perturbation of the ATP binding site.	bind
16681	4	6230	5	NULL	NULL	0	NULL	BMS-345541	NULL		bind	NULL				IKK-2	NULL		similar allosteric sites		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_3_1450_s_234	12403772	1) BMS-345541 binds to the ATP binding site of IKK-1 but not of IKK-2, or 2) BMS-345541 binds to similar allosteric sites on IKK-1 and IKK-2, but binding to the allosteric site on IKK-2 leads to a conformational change in the enzyme that alters the peptide binding site whereas the conformational change that occurs upon binding of BMS-345541 to the corresponding site on IKK-1 causes a perturbation of the ATP binding site.	bind
16682	5	6230	5	10	NULL	0	NULL	statement 4	NULL		leads to	NULL				IKK-2	NULL	conformational change of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_3_1450_s_234	12403772	1) BMS-345541 binds to the ATP binding site of IKK-1 but not of IKK-2, or 2) BMS-345541 binds to similar allosteric sites on IKK-1 and IKK-2, but binding to the allosteric site on IKK-2 leads to a conformational change in the enzyme that alters the peptide binding site whereas the conformational change that occurs upon binding of BMS-345541 to the corresponding site on IKK-1 causes a perturbation of the ATP binding site.	bind
16683	6	6230	5	NULL	NULL	0	NULL	statement 5	NULL		alters	NULL					NULL		peptide binding site		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_3_1450_s_234	12403772	1) BMS-345541 binds to the ATP binding site of IKK-1 but not of IKK-2, or 2) BMS-345541 binds to similar allosteric sites on IKK-1 and IKK-2, but binding to the allosteric site on IKK-2 leads to a conformational change in the enzyme that alters the peptide binding site whereas the conformational change that occurs upon binding of BMS-345541 to the corresponding site on IKK-1 causes a perturbation of the ATP binding site.	bind
16684	7	6230	5	10	NULL	0	NULL	statement 3	NULL		leads to	NULL				IKK-1	NULL	conformational change of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_3_1450_s_234	12403772	1) BMS-345541 binds to the ATP binding site of IKK-1 but not of IKK-2, or 2) BMS-345541 binds to similar allosteric sites on IKK-1 and IKK-2, but binding to the allosteric site on IKK-2 leads to a conformational change in the enzyme that alters the peptide binding site whereas the conformational change that occurs upon binding of BMS-345541 to the corresponding site on IKK-1 causes a perturbation of the ATP binding site.	bind
16685	8	6230	5	NULL	NULL	0	NULL	statement 7	NULL		causes	NULL				perturbation	NULL		ATP binding site		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_3_1450_s_234	12403772	1) BMS-345541 binds to the ATP binding site of IKK-1 but not of IKK-2, or 2) BMS-345541 binds to similar allosteric sites on IKK-1 and IKK-2, but binding to the allosteric site on IKK-2 leads to a conformational change in the enzyme that alters the peptide binding site whereas the conformational change that occurs upon binding of BMS-345541 to the corresponding site on IKK-1 causes a perturbation of the ATP binding site.	bind
21093	1	6230	7	NULL	NULL	NULL	NULL	BMS-345541	Chemical		binds					IKK-1	GP		ATP binding site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_3_1450_s_234	12403772	1) BMS-345541 binds to the ATP binding site of IKK-1 but not of IKK-2, or 2) BMS-345541 binds to similar allosteric sites on IKK-1 and IKK-2, but binding to the allosteric site on IKK-2 leads to a conformational change in the enzyme that alters the peptide binding site whereas the conformational change that occurs upon binding of BMS-345541 to the corresponding site on IKK-1 causes a perturbation of the ATP binding site.	bind
21094	2	6230	7	NULL	NULL	NULL	NULL	BMS-345541	Chemical		does not bind					IKK-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_3_1450_s_234	12403772	1) BMS-345541 binds to the ATP binding site of IKK-1 but not of IKK-2, or 2) BMS-345541 binds to similar allosteric sites on IKK-1 and IKK-2, but binding to the allosteric site on IKK-2 leads to a conformational change in the enzyme that alters the peptide binding site whereas the conformational change that occurs upon binding of BMS-345541 to the corresponding site on IKK-1 causes a perturbation of the ATP binding site.	bind
21095	3	6230	7	NULL	NULL	NULL	NULL	BMS-345541	Chemical		binds to					IKK-1	GP		allosteric site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_3_1450_s_234	12403772	1) BMS-345541 binds to the ATP binding site of IKK-1 but not of IKK-2, or 2) BMS-345541 binds to similar allosteric sites on IKK-1 and IKK-2, but binding to the allosteric site on IKK-2 leads to a conformational change in the enzyme that alters the peptide binding site whereas the conformational change that occurs upon binding of BMS-345541 to the corresponding site on IKK-1 causes a perturbation of the ATP binding site.	bind
21096	4	6230	7	NULL	NULL	NULL	NULL	BMS-345541	Chemical		binds to					IKK-2	GP		allosteric site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_3_1450_s_234	12403772	1) BMS-345541 binds to the ATP binding site of IKK-1 but not of IKK-2, or 2) BMS-345541 binds to similar allosteric sites on IKK-1 and IKK-2, but binding to the allosteric site on IKK-2 leads to a conformational change in the enzyme that alters the peptide binding site whereas the conformational change that occurs upon binding of BMS-345541 to the corresponding site on IKK-1 causes a perturbation of the ATP binding site.	bind
21097	5	6230	7	NULL	NULL	NULL	NULL	statement 4	Process		leads to					enzyme	GP	conformational change in the			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_3_1450_s_234	12403772	1) BMS-345541 binds to the ATP binding site of IKK-1 but not of IKK-2, or 2) BMS-345541 binds to similar allosteric sites on IKK-1 and IKK-2, but binding to the allosteric site on IKK-2 leads to a conformational change in the enzyme that alters the peptide binding site whereas the conformational change that occurs upon binding of BMS-345541 to the corresponding site on IKK-1 causes a perturbation of the ATP binding site.	bind
21098	6	6230	7	NULL	NULL	NULL	NULL	statement 4	Process		alters the 								peptide binding site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_3_1450_s_234	12403772	1) BMS-345541 binds to the ATP binding site of IKK-1 but not of IKK-2, or 2) BMS-345541 binds to similar allosteric sites on IKK-1 and IKK-2, but binding to the allosteric site on IKK-2 leads to a conformational change in the enzyme that alters the peptide binding site whereas the conformational change that occurs upon binding of BMS-345541 to the corresponding site on IKK-1 causes a perturbation of the ATP binding site.	bind
21099	7	6230	7	NULL	NULL	NULL	NULL	statement 3	Process		cause perturbation of								ATP binding site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_3_1450_s_234	12403772	1) BMS-345541 binds to the ATP binding site of IKK-1 but not of IKK-2, or 2) BMS-345541 binds to similar allosteric sites on IKK-1 and IKK-2, but binding to the allosteric site on IKK-2 leads to a conformational change in the enzyme that alters the peptide binding site whereas the conformational change that occurs upon binding of BMS-345541 to the corresponding site on IKK-1 causes a perturbation of the ATP binding site.	bind
16686	1	6231	5	NULL	NULL	0	NULL	pRNA	NULL	wt	bind	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
16687	2	6231	5	NULL	NULL	0	NULL	pRNA	NULL	wt	bind	NULL				ADP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
16688	3	6231	5	NULL	NULL	0	NULL	pRNA	NULL	wt	bind	NULL				AMP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
16689	4	6231	5	NULL	NULL	0	NULL	statement 1	NULL		higher affinity than	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
16690	5	6231	5	NULL	NULL	0	NULL	statement 1	NULL		higher affinity than	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
16691	6	6231	5	NULL	NULL	0	NULL	aptRNA	NULL		bind	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
16692	7	6231	5	NULL	NULL	0	NULL	aptRNA	NULL		bind	NULL				ADP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
16693	8	6231	5	NULL	NULL	0	NULL	aptRNA	NULL		bind	NULL				AMP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
16694	9	6231	5	NULL	NULL	0	NULL	statement 6	NULL		higher affinity than	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
16695	10	6231	5	NULL	NULL	0	NULL	statement 6	NULL		higher affinity than	NULL				statement 8	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
16696	11	6231	5	NULL	NULL	0	NULL	RNA aptamer	NULL		bind	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
16697	12	6231	5	NULL	NULL	0	NULL	RNA aptamer	NULL		bind	NULL				ADP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
16698	13	6231	5	NULL	NULL	0	NULL	RNA aptamer	NULL		bind	NULL				AMP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
16699	14	6231	5	NULL	NULL	0	NULL	RNA aptamer	NULL		bind	NULL				adenosine	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
16700	15	6231	5	NULL	NULL	0	NULL	statement 11	NULL		equal affinity to	NULL				statement 12	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
16701	16	6231	5	NULL	NULL	0	NULL	statement 12	NULL		equal affinity to	NULL				statement 13	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
16702	17	6231	5	NULL	NULL	0	NULL	statement 13	NULL		equal affinity to	NULL				statement 14	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
21100	1	6231	7	NULL	NULL	NULL	NULL	 pRNA	NucleicAcid	wt	binds		high affinity			ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
21101	2	6231	7	NULL	NULL	NULL	NULL	aptRNA	NucleicAcid		bind		high affinity			ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
21102	3	6231	7	NULL	NULL	NULL	NULL	pRNA	NucleicAcid	wt	bind					ADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
21103	4	6231	7	NULL	NULL	NULL	NULL	aptRNA	NucleicAcid		bind					ADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
21104	5	6231	7	NULL	NULL	NULL	NULL	 pRNA	NucleicAcid	wt	bind					AMP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
21105	6	6231	7	NULL	NULL	NULL	NULL	aptRNA	NucleicAcid		bind					AMP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
21106	7	6231	7	NULL	NULL	NULL	NULL	statement 1	Process		has higher affinity than					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
21107	8	6231	7	NULL	NULL	NULL	NULL	statement 1	Process		has higher affinity than					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
21108	9	6231	7	NULL	NULL	NULL	NULL	statement 2	Process		has higher affinity than					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
21110	10	6231	7	NULL	NULL	NULL	NULL	statement 2 	Process		has higher affinity than					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
21111	11	6231	7	NULL	NULL	NULL	NULL	RNA aptamer	NucleicAcid		binds					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
21129	12	6231	7	NULL	NULL	NULL	NULL	RNA aptamer	NucleicAcid		binds					ADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
21130	13	6231	7	NULL	NULL	NULL	NULL	RNA aptamer	NucleicAcid		binds					AMP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
21131	14	6231	7	NULL	NULL	NULL	NULL	RNA aptamer	NucleicAcid		binds					adenosine	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
21132	15	6231	7	NULL	NULL	NULL	NULL	statement 11	Process		has equal affinity as					statement 12	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
21133	16	6231	7	NULL	NULL	NULL	NULL	statement 11	Process		has equal affinity as					statement 13	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
21134	17	6231	7	NULL	NULL	NULL	NULL	statement 11	Process		has equal affinity as					statement 14	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_9_7119_s_232	12444088	1) Both pRNAwt and aptRNA have a higher affinity for ATP than for ADP and AMP, whereas the RNA aptamer binds ATP, ADP, AMP, and adenosine equally ( ).	bind
22922	1	6233	5	NULL	NULL	0	NULL	NFAT complex	NULL		bind	NULL				IL-2	NULL	human		NFAT binding sites	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20653_s_214	7657645	1) Both proteins are able to reconstitute  an NFAT complex with murine and human IL-2 NFAT binding sites in the  presence of Fos/Jun heterodimers; both also bind specifically to a  murine NFAT oligonucleotide without Fos and Jun proteins (Jain  et  al., 1992, 1993b; Yaseen  et al., 1993;   Fig. 1and  Fig. 6).	bind
22923	2	6233	5	NULL	NULL	0	NULL	NFAT complex	NULL		bind	NULL				IL-2-	NULL	murine		NFAT binding sites	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20653_s_214	7657645	1) Both proteins are able to reconstitute  an NFAT complex with murine and human IL-2 NFAT binding sites in the  presence of Fos/Jun heterodimers; both also bind specifically to a  murine NFAT oligonucleotide without Fos and Jun proteins (Jain  et  al., 1992, 1993b; Yaseen  et al., 1993;   Fig. 1and  Fig. 6).	bind
22924	3	6233	5	NULL	NULL	0	NULL	statement 1	NULL		in the presence of	NULL				Fos/Jun heterodimers	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20653_s_214	7657645	1) Both proteins are able to reconstitute  an NFAT complex with murine and human IL-2 NFAT binding sites in the  presence of Fos/Jun heterodimers; both also bind specifically to a  murine NFAT oligonucleotide without Fos and Jun proteins (Jain  et  al., 1992, 1993b; Yaseen  et al., 1993;   Fig. 1and  Fig. 6).	bind
54171	4	6233	5	10	NULL	0	NULL	statement 2			in the presence of					Fos/Jun heterodimers					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20653_s_214	7657645	1) Both proteins are able to reconstitute  an NFAT complex with murine and human IL-2 NFAT binding sites in the  presence of Fos/Jun heterodimers; both also bind specifically to a  murine NFAT oligonucleotide without Fos and Jun proteins (Jain  et  al., 1992, 1993b; Yaseen  et al., 1993;   Fig. 1and  Fig. 6).	bind
21487	1	6233	7	NULL	NULL	NULL	NULL	NFAT complex	GP		binds					 IL-2	GP	murine	NFAT binding sites		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20653_s_214	7657645	1) Both proteins are able to reconstitute  an NFAT complex with murine and human IL-2 NFAT binding sites in the  presence of Fos/Jun heterodimers; both also bind specifically to a  murine NFAT oligonucleotide without Fos and Jun proteins (Jain  et  al., 1992, 1993b; Yaseen  et al., 1993;   Fig. 1and  Fig. 6).	bind
21488	2	6233	7	NULL	NULL	NULL	NULL	NFAT complex	GP		binds					IL-2	GP	human	NFAT binding sites		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20653_s_214	7657645	1) Both proteins are able to reconstitute  an NFAT complex with murine and human IL-2 NFAT binding sites in the  presence of Fos/Jun heterodimers; both also bind specifically to a  murine NFAT oligonucleotide without Fos and Jun proteins (Jain  et  al., 1992, 1993b; Yaseen  et al., 1993;   Fig. 1and  Fig. 6).	bind
21489	3	6233	7	NULL	NULL	NULL	NULL	statement 1	Process		occur in presence of					Fos/Jun heterodimers	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20653_s_214	7657645	1) Both proteins are able to reconstitute  an NFAT complex with murine and human IL-2 NFAT binding sites in the  presence of Fos/Jun heterodimers; both also bind specifically to a  murine NFAT oligonucleotide without Fos and Jun proteins (Jain  et  al., 1992, 1993b; Yaseen  et al., 1993;   Fig. 1and  Fig. 6).	bind
21490	4	6233	7	NULL	NULL	NULL	NULL	statement 2	Process		occur in presence of					Fos/Jun heterodimers	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20653_s_214	7657645	1) Both proteins are able to reconstitute  an NFAT complex with murine and human IL-2 NFAT binding sites in the  presence of Fos/Jun heterodimers; both also bind specifically to a  murine NFAT oligonucleotide without Fos and Jun proteins (Jain  et  al., 1992, 1993b; Yaseen  et al., 1993;   Fig. 1and  Fig. 6).	bind
16720	1	6236	5	NULL	NULL	0	NULL	LTB4	NULL		bind	NULL				hBLT1	NULL	WT			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_42_41500_s_304	12902330	1) Cytoplasmic GTP content is inhibitory for the binding of LTB4 to the WT-hBLT1 but not to the mutants, as suggested by  Fig. 6; 2) intracellular signaling activates various kinases (GPCR kinase, protein kinase C, etc.) and inactivates the receptor by phosphorylating the C terminus.	bind
16721	2	6236	5	NULL	NULL	0	NULL	GTP	NULL	cytoplasmic	inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_42_41500_s_304	12902330	1) Cytoplasmic GTP content is inhibitory for the binding of LTB4 to the WT-hBLT1 but not to the mutants, as suggested by  Fig. 6; 2) intracellular signaling activates various kinases (GPCR kinase, protein kinase C, etc.) and inactivates the receptor by phosphorylating the C terminus.	bind
16729	3	6236	5	NULL	NULL	0	NULL	intracellular signaling	NULL		activates	NULL				GPCR kinase	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_42_41500_s_304	12902330	1) Cytoplasmic GTP content is inhibitory for the binding of LTB4 to the WT-hBLT1 but not to the mutants, as suggested by  Fig. 6; 2) intracellular signaling activates various kinases (GPCR kinase, protein kinase C, etc.) and inactivates the receptor by phosphorylating the C terminus.	bind
16730	4	6236	5	NULL	NULL	0	NULL	intracellular signaling	NULL		activates	NULL				protein kinase C	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_42_41500_s_304	12902330	1) Cytoplasmic GTP content is inhibitory for the binding of LTB4 to the WT-hBLT1 but not to the mutants, as suggested by  Fig. 6; 2) intracellular signaling activates various kinases (GPCR kinase, protein kinase C, etc.) and inactivates the receptor by phosphorylating the C terminus.	bind
16737	5	6236	5	NULL	NULL	0	NULL	intracellular signaling	NULL		phosphorylate	NULL				receptor	NULL		C terminus		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_42_41500_s_304	12902330	1) Cytoplasmic GTP content is inhibitory for the binding of LTB4 to the WT-hBLT1 but not to the mutants, as suggested by  Fig. 6; 2) intracellular signaling activates various kinases (GPCR kinase, protein kinase C, etc.) and inactivates the receptor by phosphorylating the C terminus.	bind
16755	6	6236	5	NULL	NULL	0	NULL	intracellular signaling	NULL		inactivate	NULL				receptor	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_42_41500_s_304	12902330	1) Cytoplasmic GTP content is inhibitory for the binding of LTB4 to the WT-hBLT1 but not to the mutants, as suggested by  Fig. 6; 2) intracellular signaling activates various kinases (GPCR kinase, protein kinase C, etc.) and inactivates the receptor by phosphorylating the C terminus.	bind
16758	7	6236	5	NULL	NULL	0	NULL	statement 5	NULL		leads to	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_42_41500_s_304	12902330	1) Cytoplasmic GTP content is inhibitory for the binding of LTB4 to the WT-hBLT1 but not to the mutants, as suggested by  Fig. 6; 2) intracellular signaling activates various kinases (GPCR kinase, protein kinase C, etc.) and inactivates the receptor by phosphorylating the C terminus.	bind
26087	8	6236	5	NULL	NULL	0	NULL	LTB4	NULL		bind	NULL				hBLT1	NULL	mutant			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_42_41500_s_304	12902330	1) Cytoplasmic GTP content is inhibitory for the binding of LTB4 to the WT-hBLT1 but not to the mutants, as suggested by  Fig. 6; 2) intracellular signaling activates various kinases (GPCR kinase, protein kinase C, etc.) and inactivates the receptor by phosphorylating the C terminus.	bind
26088	9	6236	5	NULL	NULL	0	NULL	GTP	NULL	cytoplasmic	does not inhibit	NULL				statement 8	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_42_41500_s_304	12902330	1) Cytoplasmic GTP content is inhibitory for the binding of LTB4 to the WT-hBLT1 but not to the mutants, as suggested by  Fig. 6; 2) intracellular signaling activates various kinases (GPCR kinase, protein kinase C, etc.) and inactivates the receptor by phosphorylating the C terminus.	bind
21135	1	6236	7	NULL	NULL	NULL	NULL	LTB4	GP		bind					hBLT1	GP	WT			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_42_41500_s_304	12902330	1) Cytoplasmic GTP content is inhibitory for the binding of LTB4 to the WT-hBLT1 but not to the mutants, as suggested by  Fig. 6; 2) intracellular signaling activates various kinases (GPCR kinase, protein kinase C, etc.) and inactivates the receptor by phosphorylating the C terminus.	bind
21136	2	6236	7	NULL	NULL	NULL	NULL	LTB4	GP		bind					hBLT1	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_42_41500_s_304	12902330	1) Cytoplasmic GTP content is inhibitory for the binding of LTB4 to the WT-hBLT1 but not to the mutants, as suggested by  Fig. 6; 2) intracellular signaling activates various kinases (GPCR kinase, protein kinase C, etc.) and inactivates the receptor by phosphorylating the C terminus.	bind
21137	3	6236	7	NULL	NULL	NULL	NULL	GTP	Chemical	cytoplasmic	inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_42_41500_s_304	12902330	1) Cytoplasmic GTP content is inhibitory for the binding of LTB4 to the WT-hBLT1 but not to the mutants, as suggested by  Fig. 6; 2) intracellular signaling activates various kinases (GPCR kinase, protein kinase C, etc.) and inactivates the receptor by phosphorylating the C terminus.	bind
21138	4	6236	7	NULL	NULL	NULL	NULL	GTP	Chemical	cytoplasmic	does not inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_42_41500_s_304	12902330	1) Cytoplasmic GTP content is inhibitory for the binding of LTB4 to the WT-hBLT1 but not to the mutants, as suggested by  Fig. 6; 2) intracellular signaling activates various kinases (GPCR kinase, protein kinase C, etc.) and inactivates the receptor by phosphorylating the C terminus.	bind
21139	5	6236	7	NULL	NULL	NULL	NULL	intracellular signaling	Process		activates					GPCR kinase	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_42_41500_s_304	12902330	1) Cytoplasmic GTP content is inhibitory for the binding of LTB4 to the WT-hBLT1 but not to the mutants, as suggested by  Fig. 6; 2) intracellular signaling activates various kinases (GPCR kinase, protein kinase C, etc.) and inactivates the receptor by phosphorylating the C terminus.	bind
21141	6	6236	7	NULL	NULL	NULL	NULL	intracellular signaling	Process		activates					protein kinase C	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_42_41500_s_304	12902330	1) Cytoplasmic GTP content is inhibitory for the binding of LTB4 to the WT-hBLT1 but not to the mutants, as suggested by  Fig. 6; 2) intracellular signaling activates various kinases (GPCR kinase, protein kinase C, etc.) and inactivates the receptor by phosphorylating the C terminus.	bind
21142	7	6236	7	NULL	NULL	NULL	NULL	intracellular signaling	Process		phosphorylates					receptor	GP		C terminus		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_42_41500_s_304	12902330	1) Cytoplasmic GTP content is inhibitory for the binding of LTB4 to the WT-hBLT1 but not to the mutants, as suggested by  Fig. 6; 2) intracellular signaling activates various kinases (GPCR kinase, protein kinase C, etc.) and inactivates the receptor by phosphorylating the C terminus.	bind
21143	8	6236	7	NULL	NULL	NULL	NULL	intracellular signaling	Process		inactivates					receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_42_41500_s_304	12902330	1) Cytoplasmic GTP content is inhibitory for the binding of LTB4 to the WT-hBLT1 but not to the mutants, as suggested by  Fig. 6; 2) intracellular signaling activates various kinases (GPCR kinase, protein kinase C, etc.) and inactivates the receptor by phosphorylating the C terminus.	bind
26356	9	6236	7	NULL	NULL	NULL	NULL	statement 6	Process		leads to					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_42_41500_s_304	12902330	1) Cytoplasmic GTP content is inhibitory for the binding of LTB4 to the WT-hBLT1 but not to the mutants, as suggested by  Fig. 6; 2) intracellular signaling activates various kinases (GPCR kinase, protein kinase C, etc.) and inactivates the receptor by phosphorylating the C terminus.	bind
16759	1	6237	5	NULL	NULL	0	NULL	Defensin	NULL		bind	NULL	may			endothelial cells	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_30_17650_s_64	8663495	1) Defensin may bind to endothelial cells providing novel sites to which plasminogen can bind; 2) defensin may bind to Glu- and to Lys-plasminogen directly, and the resultant complex may express novel cell binding epitopes; or 3) both mechanisms may be operative.	bind
16762	2	6237	5	10	NULL	0	NULL	statement 1	NULL		provide	NULL					NULL	novel 	plasminogen binding sites		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17650_s_64	8663495	1) Defensin may bind to endothelial cells providing novel sites to which plasminogen can bind; 2) defensin may bind to Glu- and to Lys-plasminogen directly, and the resultant complex may express novel cell binding epitopes; or 3) both mechanisms may be operative.	bind
16763	3	6237	5	10	NULL	0	NULL	Defensin	NULL		bind	NULL	may;; directly			Glu-plasminogen	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17650_s_64	8663495	1) Defensin may bind to endothelial cells providing novel sites to which plasminogen can bind; 2) defensin may bind to Glu- and to Lys-plasminogen directly, and the resultant complex may express novel cell binding epitopes; or 3) both mechanisms may be operative.	bind
16764	4	6237	5	10	NULL	0	NULL	Defensin	NULL		bind	NULL	may;; directly			Lys-plasminogen	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17650_s_64	8663495	1) Defensin may bind to endothelial cells providing novel sites to which plasminogen can bind; 2) defensin may bind to Glu- and to Lys-plasminogen directly, and the resultant complex may express novel cell binding epitopes; or 3) both mechanisms may be operative.	bind
16765	5	6237	5	10	NULL	0	NULL	statement 3	NULL		express	NULL	may			cell binding epitopes	NULL	novel 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17650_s_64	8663495	1) Defensin may bind to endothelial cells providing novel sites to which plasminogen can bind; 2) defensin may bind to Glu- and to Lys-plasminogen directly, and the resultant complex may express novel cell binding epitopes; or 3) both mechanisms may be operative.	bind
16766	6	6237	5	10	NULL	0	NULL	statement 4	NULL		express	NULL	may			cell binding epitopes	NULL	novel 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17650_s_64	8663495	1) Defensin may bind to endothelial cells providing novel sites to which plasminogen can bind; 2) defensin may bind to Glu- and to Lys-plasminogen directly, and the resultant complex may express novel cell binding epitopes; or 3) both mechanisms may be operative.	bind
21202	1	6237	7	NULL	NULL	NULL	NULL	Defensin	GP		bind		may			endothelial cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17650_s_64	8663495	1) Defensin may bind to endothelial cells providing novel sites to which plasminogen can bind; 2) defensin may bind to Glu- and to Lys-plasminogen directly, and the resultant complex may express novel cell binding epitopes; or 3) both mechanisms may be operative.	bind
21203	2	6237	7	NULL	NULL	NULL	NULL	statement 1	Process		provide					novel sites	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17650_s_64	8663495	1) Defensin may bind to endothelial cells providing novel sites to which plasminogen can bind; 2) defensin may bind to Glu- and to Lys-plasminogen directly, and the resultant complex may express novel cell binding epitopes; or 3) both mechanisms may be operative.	bind
21204	3	6237	7	NULL	NULL	NULL	NULL	plasminogen	GP		bind					novel sites	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17650_s_64	8663495	1) Defensin may bind to endothelial cells providing novel sites to which plasminogen can bind; 2) defensin may bind to Glu- and to Lys-plasminogen directly, and the resultant complex may express novel cell binding epitopes; or 3) both mechanisms may be operative.	bind
21205	4	6237	7	NULL	NULL	NULL	NULL	defensin	GP		bind		directly			plasminogen	GP		Glu		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17650_s_64	8663495	1) Defensin may bind to endothelial cells providing novel sites to which plasminogen can bind; 2) defensin may bind to Glu- and to Lys-plasminogen directly, and the resultant complex may express novel cell binding epitopes; or 3) both mechanisms may be operative.	bind
21206	5	6237	7	NULL	NULL	NULL	NULL	defensin	GP		bind		directly			plasminogen	GP		Lys		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17650_s_64	8663495	1) Defensin may bind to endothelial cells providing novel sites to which plasminogen can bind; 2) defensin may bind to Glu- and to Lys-plasminogen directly, and the resultant complex may express novel cell binding epitopes; or 3) both mechanisms may be operative.	bind
21207	6	6237	7	NULL	NULL	NULL	NULL	statement 4	Process		express					cell binding epitopes	CellComponent	novel			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17650_s_64	8663495	1) Defensin may bind to endothelial cells providing novel sites to which plasminogen can bind; 2) defensin may bind to Glu- and to Lys-plasminogen directly, and the resultant complex may express novel cell binding epitopes; or 3) both mechanisms may be operative.	bind
21208	7	6237	7	NULL	NULL	NULL	NULL	statement 5	Process		express					cell binding epitopes	CellComponent	novel 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17650_s_64	8663495	1) Defensin may bind to endothelial cells providing novel sites to which plasminogen can bind; 2) defensin may bind to Glu- and to Lys-plasminogen directly, and the resultant complex may express novel cell binding epitopes; or 3) both mechanisms may be operative.	bind
16767	1	6238	5	NULL	NULL	0	NULL	dIgA	NULL		bind	NULL				pIgR	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_9_4_901_s_171	9529387	1) Does the binding of dIgA to pIgR dimerize the pIgR?	bind
21209	1	6238	7	NULL	NULL	NULL	NULL	dIgA	GP		bind					pIgR 	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_4_901_s_171	9529387	1) Does the binding of dIgA to pIgR dimerize the pIgR?	bind
16740	1	6240	5	NULL	NULL	0	NULL	GPIb-IX	NULL		mediate	NULL				integrin alphaIIbbeta3	NULL	activation of			NULL	in a reconstituted CHO cell expression model	0	NULL	NULL	NULL	gw60_jbiolchem_276_45_42226_s_193	11522789	1) Dominant negative mutants of MAP kinase pathway, Raf301 and MEK1 M97K, inhibited GPIb-IX-mediated activation of integrin alphaIIbbeta3 in a reconstituted CHO cell expression model; 2) MEK inhibitors PD98059 and U0126 inhibited vWF and low dose thrombin-induced, integrin-dependent platelet aggregation in platelets in a cyclooxygenase-independent manner; and 3) vWF binding to GPIb-IX induced phosphorylation of ERK2 at the Thr-Glu-Tyr sequence, indicating that the ERK MAPK pathway is activated.	bind
16741	2	6240	5	NULL	NULL	0	NULL	Raf301	NULL	dominant negative mutants	inhibit	NULL				statement 1	NULL				NULL	in a reconstituted CHO cell expression model	0	NULL	NULL	NULL	gw60_jbiolchem_276_45_42226_s_193	11522789	1) Dominant negative mutants of MAP kinase pathway, Raf301 and MEK1 M97K, inhibited GPIb-IX-mediated activation of integrin alphaIIbbeta3 in a reconstituted CHO cell expression model; 2) MEK inhibitors PD98059 and U0126 inhibited vWF and low dose thrombin-induced, integrin-dependent platelet aggregation in platelets in a cyclooxygenase-independent manner; and 3) vWF binding to GPIb-IX induced phosphorylation of ERK2 at the Thr-Glu-Tyr sequence, indicating that the ERK MAPK pathway is activated.	bind
16742	3	6240	5	NULL	NULL	0	NULL	MEK1	NULL	dominant negative mutants	inhibit	NULL		M97K		statement 1	NULL				NULL	in a reconstituted CHO cell expression model	0	NULL	NULL	NULL	gw60_jbiolchem_276_45_42226_s_193	11522789	1) Dominant negative mutants of MAP kinase pathway, Raf301 and MEK1 M97K, inhibited GPIb-IX-mediated activation of integrin alphaIIbbeta3 in a reconstituted CHO cell expression model; 2) MEK inhibitors PD98059 and U0126 inhibited vWF and low dose thrombin-induced, integrin-dependent platelet aggregation in platelets in a cyclooxygenase-independent manner; and 3) vWF binding to GPIb-IX induced phosphorylation of ERK2 at the Thr-Glu-Tyr sequence, indicating that the ERK MAPK pathway is activated.	bind
16744	4	6240	5	10	NULL	0	NULL	PD98059	NULL		inhibit	NULL				vWF	NULL				NULL	in platelets	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_42226_s_193	11522789	1) Dominant negative mutants of MAP kinase pathway, Raf301 and MEK1 M97K, inhibited GPIb-IX-mediated activation of integrin alphaIIbbeta3 in a reconstituted CHO cell expression model; 2) MEK inhibitors PD98059 and U0126 inhibited vWF and low dose thrombin-induced, integrin-dependent platelet aggregation in platelets in a cyclooxygenase-independent manner; and 3) vWF binding to GPIb-IX induced phosphorylation of ERK2 at the Thr-Glu-Tyr sequence, indicating that the ERK MAPK pathway is activated.	bind
16745	5	6240	5	NULL	NULL	0	NULL	statement 4	NULL		is independent of	NULL				cyclooxygenase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_45_42226_s_193	11522789	1) Dominant negative mutants of MAP kinase pathway, Raf301 and MEK1 M97K, inhibited GPIb-IX-mediated activation of integrin alphaIIbbeta3 in a reconstituted CHO cell expression model; 2) MEK inhibitors PD98059 and U0126 inhibited vWF and low dose thrombin-induced, integrin-dependent platelet aggregation in platelets in a cyclooxygenase-independent manner; and 3) vWF binding to GPIb-IX induced phosphorylation of ERK2 at the Thr-Glu-Tyr sequence, indicating that the ERK MAPK pathway is activated.	bind
16746	6	6240	5	10	NULL	0	NULL	U0126	NULL		inhibit	NULL				platelet aggregation	NULL	low dose thrombin-induced, integrin-dependent			NULL	in platelets	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_42226_s_193	11522789	1) Dominant negative mutants of MAP kinase pathway, Raf301 and MEK1 M97K, inhibited GPIb-IX-mediated activation of integrin alphaIIbbeta3 in a reconstituted CHO cell expression model; 2) MEK inhibitors PD98059 and U0126 inhibited vWF and low dose thrombin-induced, integrin-dependent platelet aggregation in platelets in a cyclooxygenase-independent manner; and 3) vWF binding to GPIb-IX induced phosphorylation of ERK2 at the Thr-Glu-Tyr sequence, indicating that the ERK MAPK pathway is activated.	bind
16747	7	6240	5	NULL	NULL	0	NULL	statement 6	NULL		is independent of	NULL				cyclooxygenase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_45_42226_s_193	11522789	1) Dominant negative mutants of MAP kinase pathway, Raf301 and MEK1 M97K, inhibited GPIb-IX-mediated activation of integrin alphaIIbbeta3 in a reconstituted CHO cell expression model; 2) MEK inhibitors PD98059 and U0126 inhibited vWF and low dose thrombin-induced, integrin-dependent platelet aggregation in platelets in a cyclooxygenase-independent manner; and 3) vWF binding to GPIb-IX induced phosphorylation of ERK2 at the Thr-Glu-Tyr sequence, indicating that the ERK MAPK pathway is activated.	bind
16748	8	6240	5	NULL	NULL	0	NULL	vWF	NULL		bind	NULL				GPIb-IX	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_45_42226_s_193	11522789	1) Dominant negative mutants of MAP kinase pathway, Raf301 and MEK1 M97K, inhibited GPIb-IX-mediated activation of integrin alphaIIbbeta3 in a reconstituted CHO cell expression model; 2) MEK inhibitors PD98059 and U0126 inhibited vWF and low dose thrombin-induced, integrin-dependent platelet aggregation in platelets in a cyclooxygenase-independent manner; and 3) vWF binding to GPIb-IX induced phosphorylation of ERK2 at the Thr-Glu-Tyr sequence, indicating that the ERK MAPK pathway is activated.	bind
16750	9	6240	5	NULL	NULL	0	NULL	statement 8	NULL		induce	NULL				ERK2	NULL	phosphorylation of 	Thr-Glu-Tyr sequence		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_45_42226_s_193	11522789	1) Dominant negative mutants of MAP kinase pathway, Raf301 and MEK1 M97K, inhibited GPIb-IX-mediated activation of integrin alphaIIbbeta3 in a reconstituted CHO cell expression model; 2) MEK inhibitors PD98059 and U0126 inhibited vWF and low dose thrombin-induced, integrin-dependent platelet aggregation in platelets in a cyclooxygenase-independent manner; and 3) vWF binding to GPIb-IX induced phosphorylation of ERK2 at the Thr-Glu-Tyr sequence, indicating that the ERK MAPK pathway is activated.	bind
16753	10	6240	5	NULL	NULL	0	NULL	statement 9	NULL		indicate	NULL				ERK MAPK pathway	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_45_42226_s_193	11522789	1) Dominant negative mutants of MAP kinase pathway, Raf301 and MEK1 M97K, inhibited GPIb-IX-mediated activation of integrin alphaIIbbeta3 in a reconstituted CHO cell expression model; 2) MEK inhibitors PD98059 and U0126 inhibited vWF and low dose thrombin-induced, integrin-dependent platelet aggregation in platelets in a cyclooxygenase-independent manner; and 3) vWF binding to GPIb-IX induced phosphorylation of ERK2 at the Thr-Glu-Tyr sequence, indicating that the ERK MAPK pathway is activated.	bind
21213	1	6240	7	NULL	NULL	NULL	NULL	GPIb-IX	GP		mediates					integrin alphaIIbbeta3	GP	activation of			NULL	reconstituted CHO cell expression 	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_42226_s_193	11522789	1) Dominant negative mutants of MAP kinase pathway, Raf301 and MEK1 M97K, inhibited GPIb-IX-mediated activation of integrin alphaIIbbeta3 in a reconstituted CHO cell expression model; 2) MEK inhibitors PD98059 and U0126 inhibited vWF and low dose thrombin-induced, integrin-dependent platelet aggregation in platelets in a cyclooxygenase-independent manner; and 3) vWF binding to GPIb-IX induced phosphorylation of ERK2 at the Thr-Glu-Tyr sequence, indicating that the ERK MAPK pathway is activated.	bind
21214	2	6240	7	NULL	NULL	NULL	NULL	MAP kinase pathway	Process	Dominant negative mutants of	inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_42226_s_193	11522789	1) Dominant negative mutants of MAP kinase pathway, Raf301 and MEK1 M97K, inhibited GPIb-IX-mediated activation of integrin alphaIIbbeta3 in a reconstituted CHO cell expression model; 2) MEK inhibitors PD98059 and U0126 inhibited vWF and low dose thrombin-induced, integrin-dependent platelet aggregation in platelets in a cyclooxygenase-independent manner; and 3) vWF binding to GPIb-IX induced phosphorylation of ERK2 at the Thr-Glu-Tyr sequence, indicating that the ERK MAPK pathway is activated.	bind
21215	3	6240	7	NULL	NULL	NULL	NULL	Raf301	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_42226_s_193	11522789	1) Dominant negative mutants of MAP kinase pathway, Raf301 and MEK1 M97K, inhibited GPIb-IX-mediated activation of integrin alphaIIbbeta3 in a reconstituted CHO cell expression model; 2) MEK inhibitors PD98059 and U0126 inhibited vWF and low dose thrombin-induced, integrin-dependent platelet aggregation in platelets in a cyclooxygenase-independent manner; and 3) vWF binding to GPIb-IX induced phosphorylation of ERK2 at the Thr-Glu-Tyr sequence, indicating that the ERK MAPK pathway is activated.	bind
21216	4	6240	7	NULL	NULL	NULL	NULL	MEK1 M97K	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_42226_s_193	11522789	1) Dominant negative mutants of MAP kinase pathway, Raf301 and MEK1 M97K, inhibited GPIb-IX-mediated activation of integrin alphaIIbbeta3 in a reconstituted CHO cell expression model; 2) MEK inhibitors PD98059 and U0126 inhibited vWF and low dose thrombin-induced, integrin-dependent platelet aggregation in platelets in a cyclooxygenase-independent manner; and 3) vWF binding to GPIb-IX induced phosphorylation of ERK2 at the Thr-Glu-Tyr sequence, indicating that the ERK MAPK pathway is activated.	bind
21217	5	6240	7	NULL	NULL	NULL	NULL	PD98059	Chemical		inhibits					 vWF	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_42226_s_193	11522789	1) Dominant negative mutants of MAP kinase pathway, Raf301 and MEK1 M97K, inhibited GPIb-IX-mediated activation of integrin alphaIIbbeta3 in a reconstituted CHO cell expression model; 2) MEK inhibitors PD98059 and U0126 inhibited vWF and low dose thrombin-induced, integrin-dependent platelet aggregation in platelets in a cyclooxygenase-independent manner; and 3) vWF binding to GPIb-IX induced phosphorylation of ERK2 at the Thr-Glu-Tyr sequence, indicating that the ERK MAPK pathway is activated.	bind
21218	6	6240	7	NULL	NULL	NULL	NULL	 U0126 	Chemical		inhibits					vWF	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_42226_s_193	11522789	1) Dominant negative mutants of MAP kinase pathway, Raf301 and MEK1 M97K, inhibited GPIb-IX-mediated activation of integrin alphaIIbbeta3 in a reconstituted CHO cell expression model; 2) MEK inhibitors PD98059 and U0126 inhibited vWF and low dose thrombin-induced, integrin-dependent platelet aggregation in platelets in a cyclooxygenase-independent manner; and 3) vWF binding to GPIb-IX induced phosphorylation of ERK2 at the Thr-Glu-Tyr sequence, indicating that the ERK MAPK pathway is activated.	bind
21219	9	6240	7	NULL	NULL	NULL	NULL	PD98059	Chemical		inhibits					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_42226_s_193	11522789	1) Dominant negative mutants of MAP kinase pathway, Raf301 and MEK1 M97K, inhibited GPIb-IX-mediated activation of integrin alphaIIbbeta3 in a reconstituted CHO cell expression model; 2) MEK inhibitors PD98059 and U0126 inhibited vWF and low dose thrombin-induced, integrin-dependent platelet aggregation in platelets in a cyclooxygenase-independent manner; and 3) vWF binding to GPIb-IX induced phosphorylation of ERK2 at the Thr-Glu-Tyr sequence, indicating that the ERK MAPK pathway is activated.	bind
21220	10	6240	7	NULL	NULL	NULL	NULL	PD98059	Chemical		inhibits					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_42226_s_193	11522789	1) Dominant negative mutants of MAP kinase pathway, Raf301 and MEK1 M97K, inhibited GPIb-IX-mediated activation of integrin alphaIIbbeta3 in a reconstituted CHO cell expression model; 2) MEK inhibitors PD98059 and U0126 inhibited vWF and low dose thrombin-induced, integrin-dependent platelet aggregation in platelets in a cyclooxygenase-independent manner; and 3) vWF binding to GPIb-IX induced phosphorylation of ERK2 at the Thr-Glu-Tyr sequence, indicating that the ERK MAPK pathway is activated.	bind
21221	13	6240	7	NULL	NULL	NULL	NULL	statement 9	Process		is independent of					cyclooxygenase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_42226_s_193	11522789	1) Dominant negative mutants of MAP kinase pathway, Raf301 and MEK1 M97K, inhibited GPIb-IX-mediated activation of integrin alphaIIbbeta3 in a reconstituted CHO cell expression model; 2) MEK inhibitors PD98059 and U0126 inhibited vWF and low dose thrombin-induced, integrin-dependent platelet aggregation in platelets in a cyclooxygenase-independent manner; and 3) vWF binding to GPIb-IX induced phosphorylation of ERK2 at the Thr-Glu-Tyr sequence, indicating that the ERK MAPK pathway is activated.	bind
21223	14	6240	7	NULL	NULL	NULL	NULL	statement 10	Process		is independent of					cyclooxygenase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_42226_s_193	11522789	1) Dominant negative mutants of MAP kinase pathway, Raf301 and MEK1 M97K, inhibited GPIb-IX-mediated activation of integrin alphaIIbbeta3 in a reconstituted CHO cell expression model; 2) MEK inhibitors PD98059 and U0126 inhibited vWF and low dose thrombin-induced, integrin-dependent platelet aggregation in platelets in a cyclooxygenase-independent manner; and 3) vWF binding to GPIb-IX induced phosphorylation of ERK2 at the Thr-Glu-Tyr sequence, indicating that the ERK MAPK pathway is activated.	bind
21225	17	6240	7	NULL	NULL	NULL	NULL	vWF	GP		bind					GPIb-IX	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_42226_s_193	11522789	1) Dominant negative mutants of MAP kinase pathway, Raf301 and MEK1 M97K, inhibited GPIb-IX-mediated activation of integrin alphaIIbbeta3 in a reconstituted CHO cell expression model; 2) MEK inhibitors PD98059 and U0126 inhibited vWF and low dose thrombin-induced, integrin-dependent platelet aggregation in platelets in a cyclooxygenase-independent manner; and 3) vWF binding to GPIb-IX induced phosphorylation of ERK2 at the Thr-Glu-Tyr sequence, indicating that the ERK MAPK pathway is activated.	bind
21226	18	6240	7	NULL	NULL	NULL	NULL	statement 17	Process		induce					ERK2	GP	phosphorylation of	at the Thr-Glu-Tyr sequence		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_42226_s_193	11522789	1) Dominant negative mutants of MAP kinase pathway, Raf301 and MEK1 M97K, inhibited GPIb-IX-mediated activation of integrin alphaIIbbeta3 in a reconstituted CHO cell expression model; 2) MEK inhibitors PD98059 and U0126 inhibited vWF and low dose thrombin-induced, integrin-dependent platelet aggregation in platelets in a cyclooxygenase-independent manner; and 3) vWF binding to GPIb-IX induced phosphorylation of ERK2 at the Thr-Glu-Tyr sequence, indicating that the ERK MAPK pathway is activated.	bind
21231	19	6240	7	NULL	NULL	NULL	NULL	statement 18	Process		indicate					ERK MAPK pathway	Process	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_42226_s_193	11522789	1) Dominant negative mutants of MAP kinase pathway, Raf301 and MEK1 M97K, inhibited GPIb-IX-mediated activation of integrin alphaIIbbeta3 in a reconstituted CHO cell expression model; 2) MEK inhibitors PD98059 and U0126 inhibited vWF and low dose thrombin-induced, integrin-dependent platelet aggregation in platelets in a cyclooxygenase-independent manner; and 3) vWF binding to GPIb-IX induced phosphorylation of ERK2 at the Thr-Glu-Tyr sequence, indicating that the ERK MAPK pathway is activated.	bind
45566	8	6240	7	NULL	NULL	NULL	NULL	platelet aggregation	Process		depends on					integrin	GP				NULL	platelets	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_42226_s_193	11522789	1) Dominant negative mutants of MAP kinase pathway, Raf301 and MEK1 M97K, inhibited GPIb-IX-mediated activation of integrin alphaIIbbeta3 in a reconstituted CHO cell expression model; 2) MEK inhibitors PD98059 and U0126 inhibited vWF and low dose thrombin-induced, integrin-dependent platelet aggregation in platelets in a cyclooxygenase-independent manner; and 3) vWF binding to GPIb-IX induced phosphorylation of ERK2 at the Thr-Glu-Tyr sequence, indicating that the ERK MAPK pathway is activated.	bind
45567	7	6240	7	NULL	NULL	NULL	NULL	thrombin	GP		induce					platelet aggregation	Process				NULL	platelets	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_42226_s_193	11522789	1) Dominant negative mutants of MAP kinase pathway, Raf301 and MEK1 M97K, inhibited GPIb-IX-mediated activation of integrin alphaIIbbeta3 in a reconstituted CHO cell expression model; 2) MEK inhibitors PD98059 and U0126 inhibited vWF and low dose thrombin-induced, integrin-dependent platelet aggregation in platelets in a cyclooxygenase-independent manner; and 3) vWF binding to GPIb-IX induced phosphorylation of ERK2 at the Thr-Glu-Tyr sequence, indicating that the ERK MAPK pathway is activated.	bind
45568	11	6240	7	NULL	NULL	NULL	NULL	U0126	Chemical		inhibits					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_42226_s_193	11522789	1) Dominant negative mutants of MAP kinase pathway, Raf301 and MEK1 M97K, inhibited GPIb-IX-mediated activation of integrin alphaIIbbeta3 in a reconstituted CHO cell expression model; 2) MEK inhibitors PD98059 and U0126 inhibited vWF and low dose thrombin-induced, integrin-dependent platelet aggregation in platelets in a cyclooxygenase-independent manner; and 3) vWF binding to GPIb-IX induced phosphorylation of ERK2 at the Thr-Glu-Tyr sequence, indicating that the ERK MAPK pathway is activated.	bind
45569	12	6240	7	NULL	NULL	NULL	NULL	U0126	Chemical		inhibits					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_42226_s_193	11522789	1) Dominant negative mutants of MAP kinase pathway, Raf301 and MEK1 M97K, inhibited GPIb-IX-mediated activation of integrin alphaIIbbeta3 in a reconstituted CHO cell expression model; 2) MEK inhibitors PD98059 and U0126 inhibited vWF and low dose thrombin-induced, integrin-dependent platelet aggregation in platelets in a cyclooxygenase-independent manner; and 3) vWF binding to GPIb-IX induced phosphorylation of ERK2 at the Thr-Glu-Tyr sequence, indicating that the ERK MAPK pathway is activated.	bind
45570	15	6240	7	NULL	NULL	NULL	NULL	statement 11	Process		is independent of					cyclooxygenase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_42226_s_193	11522789	1) Dominant negative mutants of MAP kinase pathway, Raf301 and MEK1 M97K, inhibited GPIb-IX-mediated activation of integrin alphaIIbbeta3 in a reconstituted CHO cell expression model; 2) MEK inhibitors PD98059 and U0126 inhibited vWF and low dose thrombin-induced, integrin-dependent platelet aggregation in platelets in a cyclooxygenase-independent manner; and 3) vWF binding to GPIb-IX induced phosphorylation of ERK2 at the Thr-Glu-Tyr sequence, indicating that the ERK MAPK pathway is activated.	bind
45571	16	6240	7	NULL	NULL	NULL	NULL	statement 12	Process		is independent of					cyclooxygenase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_42226_s_193	11522789	1) Dominant negative mutants of MAP kinase pathway, Raf301 and MEK1 M97K, inhibited GPIb-IX-mediated activation of integrin alphaIIbbeta3 in a reconstituted CHO cell expression model; 2) MEK inhibitors PD98059 and U0126 inhibited vWF and low dose thrombin-induced, integrin-dependent platelet aggregation in platelets in a cyclooxygenase-independent manner; and 3) vWF binding to GPIb-IX induced phosphorylation of ERK2 at the Thr-Glu-Tyr sequence, indicating that the ERK MAPK pathway is activated.	bind
16768	1	6241	5	10	NULL	0	NULL	VIP			bind					VPAC2 receptor					NULL	during some stages of brain development	NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_314_2_745_s_184	15872042	1) During some stages of brain development, the binding of VIP or PACAP to VPAC2 receptors leads to activation of separate transduction pathways.	bind
16769	2	6241	5	10	NULL	0	NULL	PACAP			bind					VPAC2 receptor					NULL	during some stages of brain development	NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_314_2_745_s_184	15872042	1) During some stages of brain development, the binding of VIP or PACAP to VPAC2 receptors leads to activation of separate transduction pathways.	bind
16770	3	6241	5	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				separate transduction pathways	NULL	activation of			NULL	during some stages of brain development	0	NULL	NULL	NULL	gw70_jpharmacolexpther_314_2_745_s_184	15872042	1) During some stages of brain development, the binding of VIP or PACAP to VPAC2 receptors leads to activation of separate transduction pathways.	bind
16771	4	6241	5	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				separate transduction pathways	NULL	activation of			NULL	during some stages of brain development	0	NULL	NULL	NULL	gw70_jpharmacolexpther_314_2_745_s_184	15872042	1) During some stages of brain development, the binding of VIP or PACAP to VPAC2 receptors leads to activation of separate transduction pathways.	bind
54172	5	6241	5	10	NULL	0	NULL	statement 1			is an alternative to					statement 2					NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_314_2_745_s_184	15872042	1) During some stages of brain development, the binding of VIP or PACAP to VPAC2 receptors leads to activation of separate transduction pathways.	bind
21232	1	6241	7	NULL	NULL	NULL	NULL	VIP	GP		bind					VPAC2 receptors	GP				NULL	during stages of brain development	NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_314_2_745_s_184	15872042	1) During some stages of brain development, the binding of VIP or PACAP to VPAC2 receptors leads to activation of separate transduction pathways.	bind
21233	2	6241	7	NULL	NULL	NULL	NULL	PACAP	GP		bind					VPAC2 receptors	GP				NULL	during stages of brain development	NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_314_2_745_s_184	15872042	1) During some stages of brain development, the binding of VIP or PACAP to VPAC2 receptors leads to activation of separate transduction pathways.	bind
21234	3	6241	7	NULL	NULL	NULL	NULL	statement 1	Process		leads to					transduction pathways	Process	activation of			NULL	during stages of brain development	NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_314_2_745_s_184	15872042	1) During some stages of brain development, the binding of VIP or PACAP to VPAC2 receptors leads to activation of separate transduction pathways.	bind
21235	4	6241	7	NULL	NULL	NULL	NULL	statement 2	Process		leads to					transduction pathways	Process	activation of			NULL	during stages of brain development	NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_314_2_745_s_184	15872042	1) During some stages of brain development, the binding of VIP or PACAP to VPAC2 receptors leads to activation of separate transduction pathways.	bind
21236	5	6241	7	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_314_2_745_s_184	15872042	1) During some stages of brain development, the binding of VIP or PACAP to VPAC2 receptors leads to activation of separate transduction pathways.	bind
16773	1	6242	5	10	NULL	0	NULL	iron			is associated with					high molecular weight fraction					NULL	in phloem	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25062_s_259	11983700	1) Essentially all iron in the phloem is associated with the high molecular weight fraction; 2) ITP-iron complexes rapidly appear in pure phloem exudate after feeding of cotyledons with 55Fe; 3) ITP carries iron  in vivo and is able to bind additional iron  in vitro; 4) purified ITP binds preferentially Fe3+, the dominant iron species in the phloem; and 5) the amino acid sequence of ITP suggests it is capable of binding several metal ions per molecule.	bind
16776	2	6242	5	NULL	NULL	0	NULL	cotyledons	NULL		fed with	NULL				55Fe	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_28_25062_s_259	11983700	1) Essentially all iron in the phloem is associated with the high molecular weight fraction; 2) ITP-iron complexes rapidly appear in pure phloem exudate after feeding of cotyledons with 55Fe; 3) ITP carries iron  in vivo and is able to bind additional iron  in vitro; 4) purified ITP binds preferentially Fe3+, the dominant iron species in the phloem; and 5) the amino acid sequence of ITP suggests it is capable of binding several metal ions per molecule.	bind
16778	3	6242	5	NULL	NULL	0	NULL	ITP-iron complexes	NULL		appear in	NULL	rapidly			phloem exudate	NULL	pure			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25062_s_259	11983700	1) Essentially all iron in the phloem is associated with the high molecular weight fraction; 2) ITP-iron complexes rapidly appear in pure phloem exudate after feeding of cotyledons with 55Fe; 3) ITP carries iron  in vivo and is able to bind additional iron  in vitro; 4) purified ITP binds preferentially Fe3+, the dominant iron species in the phloem; and 5) the amino acid sequence of ITP suggests it is capable of binding several metal ions per molecule.	bind
16779	4	6242	5	NULL	NULL	0	NULL	statement 3	NULL		occurs after	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_28_25062_s_259	11983700	1) Essentially all iron in the phloem is associated with the high molecular weight fraction; 2) ITP-iron complexes rapidly appear in pure phloem exudate after feeding of cotyledons with 55Fe; 3) ITP carries iron  in vivo and is able to bind additional iron  in vitro; 4) purified ITP binds preferentially Fe3+, the dominant iron species in the phloem; and 5) the amino acid sequence of ITP suggests it is capable of binding several metal ions per molecule.	bind
16781	5	6242	5	NULL	NULL	0	NULL	ITP	NULL		carries	NULL				iron	NULL				NULL	in vivo	0	NULL	NULL	NULL	gw60_jbiolchem_277_28_25062_s_259	11983700	1) Essentially all iron in the phloem is associated with the high molecular weight fraction; 2) ITP-iron complexes rapidly appear in pure phloem exudate after feeding of cotyledons with 55Fe; 3) ITP carries iron  in vivo and is able to bind additional iron  in vitro; 4) purified ITP binds preferentially Fe3+, the dominant iron species in the phloem; and 5) the amino acid sequence of ITP suggests it is capable of binding several metal ions per molecule.	bind
16783	6	6242	5	NULL	NULL	0	NULL	ITP	NULL		bind	NULL				iron	NULL	additional			NULL	in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_277_28_25062_s_259	11983700	1) Essentially all iron in the phloem is associated with the high molecular weight fraction; 2) ITP-iron complexes rapidly appear in pure phloem exudate after feeding of cotyledons with 55Fe; 3) ITP carries iron  in vivo and is able to bind additional iron  in vitro; 4) purified ITP binds preferentially Fe3+, the dominant iron species in the phloem; and 5) the amino acid sequence of ITP suggests it is capable of binding several metal ions per molecule.	bind
16784	7	6242	5	NULL	NULL	0	NULL	ITP	NULL	purified	bind	NULL	preferentially			Fe3+	NULL				NULL	in phloem	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25062_s_259	11983700	1) Essentially all iron in the phloem is associated with the high molecular weight fraction; 2) ITP-iron complexes rapidly appear in pure phloem exudate after feeding of cotyledons with 55Fe; 3) ITP carries iron  in vivo and is able to bind additional iron  in vitro; 4) purified ITP binds preferentially Fe3+, the dominant iron species in the phloem; and 5) the amino acid sequence of ITP suggests it is capable of binding several metal ions per molecule.	bind
16785	8	6242	5	NULL	NULL	0	NULL	Fe3+	NULL		is	NULL				dominant iron species	NULL				NULL	in phloem	0	NULL	NULL	NULL	gw60_jbiolchem_277_28_25062_s_259	11983700	1) Essentially all iron in the phloem is associated with the high molecular weight fraction; 2) ITP-iron complexes rapidly appear in pure phloem exudate after feeding of cotyledons with 55Fe; 3) ITP carries iron  in vivo and is able to bind additional iron  in vitro; 4) purified ITP binds preferentially Fe3+, the dominant iron species in the phloem; and 5) the amino acid sequence of ITP suggests it is capable of binding several metal ions per molecule.	bind
16786	9	6242	5	NULL	NULL	0	NULL	ITP	NULL		bind	NULL				metal ions per molecule	NULL	several			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_28_25062_s_259	11983700	1) Essentially all iron in the phloem is associated with the high molecular weight fraction; 2) ITP-iron complexes rapidly appear in pure phloem exudate after feeding of cotyledons with 55Fe; 3) ITP carries iron  in vivo and is able to bind additional iron  in vitro; 4) purified ITP binds preferentially Fe3+, the dominant iron species in the phloem; and 5) the amino acid sequence of ITP suggests it is capable of binding several metal ions per molecule.	bind
16787	10	6242	5	NULL	NULL	0	NULL	ITP	NULL	amino acid sequence	suggest	NULL				statement 9	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_28_25062_s_259	11983700	1) Essentially all iron in the phloem is associated with the high molecular weight fraction; 2) ITP-iron complexes rapidly appear in pure phloem exudate after feeding of cotyledons with 55Fe; 3) ITP carries iron  in vivo and is able to bind additional iron  in vitro; 4) purified ITP binds preferentially Fe3+, the dominant iron species in the phloem; and 5) the amino acid sequence of ITP suggests it is capable of binding several metal ions per molecule.	bind
21237	1	6242	7	NULL	NULL	NULL	NULL	ITP-iron complex	GP		appear in		rapidly			 phloem exudate	OrganismPart	pure			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25062_s_259	11983700	1) Essentially all iron in the phloem is associated with the high molecular weight fraction; 2) ITP-iron complexes rapidly appear in pure phloem exudate after feeding of cotyledons with 55Fe; 3) ITP carries iron  in vivo and is able to bind additional iron  in vitro; 4) purified ITP binds preferentially Fe3+, the dominant iron species in the phloem; and 5) the amino acid sequence of ITP suggests it is capable of binding several metal ions per molecule.	bind
21238	2	6242	7	NULL	NULL	NULL	NULL	cotyledons	OrganismPart		fed with					 Fe	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25062_s_259	11983700	1) Essentially all iron in the phloem is associated with the high molecular weight fraction; 2) ITP-iron complexes rapidly appear in pure phloem exudate after feeding of cotyledons with 55Fe; 3) ITP carries iron  in vivo and is able to bind additional iron  in vitro; 4) purified ITP binds preferentially Fe3+, the dominant iron species in the phloem; and 5) the amino acid sequence of ITP suggests it is capable of binding several metal ions per molecule.	bind
21239	3	6242	7	NULL	NULL	NULL	NULL	ITP	GP		carries					iron	Chemical				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25062_s_259	11983700	1) Essentially all iron in the phloem is associated with the high molecular weight fraction; 2) ITP-iron complexes rapidly appear in pure phloem exudate after feeding of cotyledons with 55Fe; 3) ITP carries iron  in vivo and is able to bind additional iron  in vitro; 4) purified ITP binds preferentially Fe3+, the dominant iron species in the phloem; and 5) the amino acid sequence of ITP suggests it is capable of binding several metal ions per molecule.	bind
21240	4	6242	7	NULL	NULL	NULL	NULL	statement 3	Process		binds					iron	Chemical				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25062_s_259	11983700	1) Essentially all iron in the phloem is associated with the high molecular weight fraction; 2) ITP-iron complexes rapidly appear in pure phloem exudate after feeding of cotyledons with 55Fe; 3) ITP carries iron  in vivo and is able to bind additional iron  in vitro; 4) purified ITP binds preferentially Fe3+, the dominant iron species in the phloem; and 5) the amino acid sequence of ITP suggests it is capable of binding several metal ions per molecule.	bind
21241	5	6242	7	NULL	NULL	NULL	NULL	ITP	GP	purified	binds		preferentially			Fe3+	Chemical				NULL	in the phloem	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25062_s_259	11983700	1) Essentially all iron in the phloem is associated with the high molecular weight fraction; 2) ITP-iron complexes rapidly appear in pure phloem exudate after feeding of cotyledons with 55Fe; 3) ITP carries iron  in vivo and is able to bind additional iron  in vitro; 4) purified ITP binds preferentially Fe3+, the dominant iron species in the phloem; and 5) the amino acid sequence of ITP suggests it is capable of binding several metal ions per molecule.	bind
21242	6	6242	7	NULL	NULL	NULL	NULL	ITP 	GP		bind					metal ions 	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25062_s_259	11983700	1) Essentially all iron in the phloem is associated with the high molecular weight fraction; 2) ITP-iron complexes rapidly appear in pure phloem exudate after feeding of cotyledons with 55Fe; 3) ITP carries iron  in vivo and is able to bind additional iron  in vitro; 4) purified ITP binds preferentially Fe3+, the dominant iron species in the phloem; and 5) the amino acid sequence of ITP suggests it is capable of binding several metal ions per molecule.	bind
21243	7	6242	7	NULL	NULL	NULL	NULL	iron	Chemical	phloem	associate with					high molecular weight fraction	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25062_s_259	11983700	1) Essentially all iron in the phloem is associated with the high molecular weight fraction; 2) ITP-iron complexes rapidly appear in pure phloem exudate after feeding of cotyledons with 55Fe; 3) ITP carries iron  in vivo and is able to bind additional iron  in vitro; 4) purified ITP binds preferentially Fe3+, the dominant iron species in the phloem; and 5) the amino acid sequence of ITP suggests it is capable of binding several metal ions per molecule.	bind
45559	8	6242	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs after					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25062_s_259	11983700	1) Essentially all iron in the phloem is associated with the high molecular weight fraction; 2) ITP-iron complexes rapidly appear in pure phloem exudate after feeding of cotyledons with 55Fe; 3) ITP carries iron  in vivo and is able to bind additional iron  in vitro; 4) purified ITP binds preferentially Fe3+, the dominant iron species in the phloem; and 5) the amino acid sequence of ITP suggests it is capable of binding several metal ions per molecule.	bind
16788	1	6243	5	NULL	NULL	0	NULL	fibrinogen	NULL		bind	NULL				alphaIIbbeta3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_28_25715_s_179	11994301	1) Expression of constitutively active Rap1b (V12) augments fibrinogen binding to alphaIIbbeta3 when megakaryocytes are stimulated through the PAR4 thrombin receptor.	bind
16789	2	6243	5	NULL	NULL	0	NULL	PAR4 thrombin receptor	NULL		stimulate	NULL				megakaryocytes	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_28_25715_s_179	11994301	1) Expression of constitutively active Rap1b (V12) augments fibrinogen binding to alphaIIbbeta3 when megakaryocytes are stimulated through the PAR4 thrombin receptor.	bind
16790	4	6243	5	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25715_s_179	11994301	1) Expression of constitutively active Rap1b (V12) augments fibrinogen binding to alphaIIbbeta3 when megakaryocytes are stimulated through the PAR4 thrombin receptor.	bind
16791	3	6243	5	10	NULL	0	NULL	Rap1b (V12)	NULL	constitutively active	augment	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25715_s_179	11994301	1) Expression of constitutively active Rap1b (V12) augments fibrinogen binding to alphaIIbbeta3 when megakaryocytes are stimulated through the PAR4 thrombin receptor.	bind
21244	1	6243	7	NULL	NULL	NULL	NULL	fibrinogen	GP		bind					 alphaIIbbeta3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25715_s_179	11994301	1) Expression of constitutively active Rap1b (V12) augments fibrinogen binding to alphaIIbbeta3 when megakaryocytes are stimulated through the PAR4 thrombin receptor.	bind
21245	2	6243	7	NULL	NULL	NULL	NULL	Rap1b (V12) 	GP	constitutively active	augments					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25715_s_179	11994301	1) Expression of constitutively active Rap1b (V12) augments fibrinogen binding to alphaIIbbeta3 when megakaryocytes are stimulated through the PAR4 thrombin receptor.	bind
21246	3	6243	7	NULL	NULL	NULL	NULL	PAR4 thrombin receptor	GP		stimulate					megakaryocytes	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25715_s_179	11994301	1) Expression of constitutively active Rap1b (V12) augments fibrinogen binding to alphaIIbbeta3 when megakaryocytes are stimulated through the PAR4 thrombin receptor.	bind
26358	4	6243	7	NULL	NULL	NULL	NULL	statement 3	Process		lead to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25715_s_179	11994301	1) Expression of constitutively active Rap1b (V12) augments fibrinogen binding to alphaIIbbeta3 when megakaryocytes are stimulated through the PAR4 thrombin receptor.	bind
16792	1	6244	5	NULL	NULL	0	NULL	5-HT4(a)	NULL		induce	NULL					NULL	activation of		SRE	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_23_20812_s_295	11923294	1) Expression of wild type Galpha13 enhanced 5-HT4(a)-induced SRE activation (Fig.  5); 2) Galpha13 was inhibited by the RGS domain of p115RhoGEF, which is specific for Galpha12 and Galpha13 (Fig.  4); 3) C3 exoenzyme, a specific inhibitor of Rho proteins, inhibited SRE activation by 5-HT4(a) (Fig.  6); 4) the above-mentioned inhibitors and dominant-negative constructs also effectively inhibited SRE activation induced by Galpha13; 5) finally, direct measurement of Rho activity using a rhotekin binding assay showed that the 5-HT4(a) receptor is able to activate Rho (Fig.  6 C).	bind
16793	2	6244	5	10	NULL	0	NULL	Galpha13	NULL	wild type	enhance	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_23_20812_s_295	11923294	1) Expression of wild type Galpha13 enhanced 5-HT4(a)-induced SRE activation (Fig.  5); 2) Galpha13 was inhibited by the RGS domain of p115RhoGEF, which is specific for Galpha12 and Galpha13 (Fig.  4); 3) C3 exoenzyme, a specific inhibitor of Rho proteins, inhibited SRE activation by 5-HT4(a) (Fig.  6); 4) the above-mentioned inhibitors and dominant-negative constructs also effectively inhibited SRE activation induced by Galpha13; 5) finally, direct measurement of Rho activity using a rhotekin binding assay showed that the 5-HT4(a) receptor is able to activate Rho (Fig.  6 C).	bind
16794	3	6244	5	NULL	NULL	0	NULL	p115RhoGEF	NULL		inhibit	NULL		RGS domain		Galpha13	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_23_20812_s_295	11923294	1) Expression of wild type Galpha13 enhanced 5-HT4(a)-induced SRE activation (Fig.  5); 2) Galpha13 was inhibited by the RGS domain of p115RhoGEF, which is specific for Galpha12 and Galpha13 (Fig.  4); 3) C3 exoenzyme, a specific inhibitor of Rho proteins, inhibited SRE activation by 5-HT4(a) (Fig.  6); 4) the above-mentioned inhibitors and dominant-negative constructs also effectively inhibited SRE activation induced by Galpha13; 5) finally, direct measurement of Rho activity using a rhotekin binding assay showed that the 5-HT4(a) receptor is able to activate Rho (Fig.  6 C).	bind
16795	4	6244	5	NULL	NULL	0	NULL	p115RhoGEF	NULL		is specific for	NULL				Galpha12	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_23_20812_s_295	11923294	1) Expression of wild type Galpha13 enhanced 5-HT4(a)-induced SRE activation (Fig.  5); 2) Galpha13 was inhibited by the RGS domain of p115RhoGEF, which is specific for Galpha12 and Galpha13 (Fig.  4); 3) C3 exoenzyme, a specific inhibitor of Rho proteins, inhibited SRE activation by 5-HT4(a) (Fig.  6); 4) the above-mentioned inhibitors and dominant-negative constructs also effectively inhibited SRE activation induced by Galpha13; 5) finally, direct measurement of Rho activity using a rhotekin binding assay showed that the 5-HT4(a) receptor is able to activate Rho (Fig.  6 C).	bind
16796	5	6244	5	NULL	NULL	0	NULL	p115RhoGEF	NULL		is specific for	NULL		RGS domain		Galpha13	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_23_20812_s_295	11923294	1) Expression of wild type Galpha13 enhanced 5-HT4(a)-induced SRE activation (Fig.  5); 2) Galpha13 was inhibited by the RGS domain of p115RhoGEF, which is specific for Galpha12 and Galpha13 (Fig.  4); 3) C3 exoenzyme, a specific inhibitor of Rho proteins, inhibited SRE activation by 5-HT4(a) (Fig.  6); 4) the above-mentioned inhibitors and dominant-negative constructs also effectively inhibited SRE activation induced by Galpha13; 5) finally, direct measurement of Rho activity using a rhotekin binding assay showed that the 5-HT4(a) receptor is able to activate Rho (Fig.  6 C).	bind
16797	6	6244	5	NULL	NULL	0	NULL	5-HT4(a)	NULL		activate	NULL					NULL			SRE	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_23_20812_s_295	11923294	1) Expression of wild type Galpha13 enhanced 5-HT4(a)-induced SRE activation (Fig.  5); 2) Galpha13 was inhibited by the RGS domain of p115RhoGEF, which is specific for Galpha12 and Galpha13 (Fig.  4); 3) C3 exoenzyme, a specific inhibitor of Rho proteins, inhibited SRE activation by 5-HT4(a) (Fig.  6); 4) the above-mentioned inhibitors and dominant-negative constructs also effectively inhibited SRE activation induced by Galpha13; 5) finally, direct measurement of Rho activity using a rhotekin binding assay showed that the 5-HT4(a) receptor is able to activate Rho (Fig.  6 C).	bind
16798	7	6244	5	10	NULL	0	NULL	C3 exoenzyme			inhibit					statement 6					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_23_20812_s_295	11923294	1) Expression of wild type Galpha13 enhanced 5-HT4(a)-induced SRE activation (Fig.  5); 2) Galpha13 was inhibited by the RGS domain of p115RhoGEF, which is specific for Galpha12 and Galpha13 (Fig.  4); 3) C3 exoenzyme, a specific inhibitor of Rho proteins, inhibited SRE activation by 5-HT4(a) (Fig.  6); 4) the above-mentioned inhibitors and dominant-negative constructs also effectively inhibited SRE activation induced by Galpha13; 5) finally, direct measurement of Rho activity using a rhotekin binding assay showed that the 5-HT4(a) receptor is able to activate Rho (Fig.  6 C).	bind
16799	8	6244	5	NULL	NULL	0	NULL	Galpha13	NULL		induce	NULL					NULL	activation of		SRE	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_23_20812_s_295	11923294	1) Expression of wild type Galpha13 enhanced 5-HT4(a)-induced SRE activation (Fig.  5); 2) Galpha13 was inhibited by the RGS domain of p115RhoGEF, which is specific for Galpha12 and Galpha13 (Fig.  4); 3) C3 exoenzyme, a specific inhibitor of Rho proteins, inhibited SRE activation by 5-HT4(a) (Fig.  6); 4) the above-mentioned inhibitors and dominant-negative constructs also effectively inhibited SRE activation induced by Galpha13; 5) finally, direct measurement of Rho activity using a rhotekin binding assay showed that the 5-HT4(a) receptor is able to activate Rho (Fig.  6 C).	bind
16800	9	6244	5	NULL	NULL	0	NULL	p115RhoGEF	NULL		inhibit	NULL	effectively			statement 8	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_23_20812_s_295	11923294	1) Expression of wild type Galpha13 enhanced 5-HT4(a)-induced SRE activation (Fig.  5); 2) Galpha13 was inhibited by the RGS domain of p115RhoGEF, which is specific for Galpha12 and Galpha13 (Fig.  4); 3) C3 exoenzyme, a specific inhibitor of Rho proteins, inhibited SRE activation by 5-HT4(a) (Fig.  6); 4) the above-mentioned inhibitors and dominant-negative constructs also effectively inhibited SRE activation induced by Galpha13; 5) finally, direct measurement of Rho activity using a rhotekin binding assay showed that the 5-HT4(a) receptor is able to activate Rho (Fig.  6 C).	bind
16801	10	6244	5	NULL	NULL	0	NULL	C3 exoenzyme	NULL		inhibit	NULL	effectively			statement 8	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_23_20812_s_295	11923294	1) Expression of wild type Galpha13 enhanced 5-HT4(a)-induced SRE activation (Fig.  5); 2) Galpha13 was inhibited by the RGS domain of p115RhoGEF, which is specific for Galpha12 and Galpha13 (Fig.  4); 3) C3 exoenzyme, a specific inhibitor of Rho proteins, inhibited SRE activation by 5-HT4(a) (Fig.  6); 4) the above-mentioned inhibitors and dominant-negative constructs also effectively inhibited SRE activation induced by Galpha13; 5) finally, direct measurement of Rho activity using a rhotekin binding assay showed that the 5-HT4(a) receptor is able to activate Rho (Fig.  6 C).	bind
16802	11	6244	5	NULL	NULL	0	NULL	5-HT4(a) receptor	NULL		activate	NULL				Rho	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_23_20812_s_295	11923294	1) Expression of wild type Galpha13 enhanced 5-HT4(a)-induced SRE activation (Fig.  5); 2) Galpha13 was inhibited by the RGS domain of p115RhoGEF, which is specific for Galpha12 and Galpha13 (Fig.  4); 3) C3 exoenzyme, a specific inhibitor of Rho proteins, inhibited SRE activation by 5-HT4(a) (Fig.  6); 4) the above-mentioned inhibitors and dominant-negative constructs also effectively inhibited SRE activation induced by Galpha13; 5) finally, direct measurement of Rho activity using a rhotekin binding assay showed that the 5-HT4(a) receptor is able to activate Rho (Fig.  6 C).	bind
54173	12	6244	5	10	NULL	0	NULL	C3 exoenzyme			is an inhibitor of		specific			Rho proteins					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_23_20812_s_295	11923294	1) Expression of wild type Galpha13 enhanced 5-HT4(a)-induced SRE activation (Fig.  5); 2) Galpha13 was inhibited by the RGS domain of p115RhoGEF, which is specific for Galpha12 and Galpha13 (Fig.  4); 3) C3 exoenzyme, a specific inhibitor of Rho proteins, inhibited SRE activation by 5-HT4(a) (Fig.  6); 4) the above-mentioned inhibitors and dominant-negative constructs also effectively inhibited SRE activation induced by Galpha13; 5) finally, direct measurement of Rho activity using a rhotekin binding assay showed that the 5-HT4(a) receptor is able to activate Rho (Fig.  6 C).	bind
21305	1	6244	7	NULL	NULL	NULL	NULL	5-HT4	Chemical		induce							activation of		 SRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_23_20812_s_295	11923294	1) Expression of wild type Galpha13 enhanced 5-HT4(a)-induced SRE activation (Fig.  5); 2) Galpha13 was inhibited by the RGS domain of p115RhoGEF, which is specific for Galpha12 and Galpha13 (Fig.  4); 3) C3 exoenzyme, a specific inhibitor of Rho proteins, inhibited SRE activation by 5-HT4(a) (Fig.  6); 4) the above-mentioned inhibitors and dominant-negative constructs also effectively inhibited SRE activation induced by Galpha13; 5) finally, direct measurement of Rho activity using a rhotekin binding assay showed that the 5-HT4(a) receptor is able to activate Rho (Fig.  6 C).	bind
21307	2	6244	7	NULL	NULL	NULL	NULL	Galpha13	GP	wild type	enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_23_20812_s_295	11923294	1) Expression of wild type Galpha13 enhanced 5-HT4(a)-induced SRE activation (Fig.  5); 2) Galpha13 was inhibited by the RGS domain of p115RhoGEF, which is specific for Galpha12 and Galpha13 (Fig.  4); 3) C3 exoenzyme, a specific inhibitor of Rho proteins, inhibited SRE activation by 5-HT4(a) (Fig.  6); 4) the above-mentioned inhibitors and dominant-negative constructs also effectively inhibited SRE activation induced by Galpha13; 5) finally, direct measurement of Rho activity using a rhotekin binding assay showed that the 5-HT4(a) receptor is able to activate Rho (Fig.  6 C).	bind
21368	3	6244	7	NULL	NULL	NULL	NULL	p115RhoGEF	GP		inhibits			RGS domain		Galpha13	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_23_20812_s_295	11923294	1) Expression of wild type Galpha13 enhanced 5-HT4(a)-induced SRE activation (Fig.  5); 2) Galpha13 was inhibited by the RGS domain of p115RhoGEF, which is specific for Galpha12 and Galpha13 (Fig.  4); 3) C3 exoenzyme, a specific inhibitor of Rho proteins, inhibited SRE activation by 5-HT4(a) (Fig.  6); 4) the above-mentioned inhibitors and dominant-negative constructs also effectively inhibited SRE activation induced by Galpha13; 5) finally, direct measurement of Rho activity using a rhotekin binding assay showed that the 5-HT4(a) receptor is able to activate Rho (Fig.  6 C).	bind
21369	4	6244	7	NULL	NULL	NULL	NULL	5-HT4	Chemical		activates									SRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_23_20812_s_295	11923294	1) Expression of wild type Galpha13 enhanced 5-HT4(a)-induced SRE activation (Fig.  5); 2) Galpha13 was inhibited by the RGS domain of p115RhoGEF, which is specific for Galpha12 and Galpha13 (Fig.  4); 3) C3 exoenzyme, a specific inhibitor of Rho proteins, inhibited SRE activation by 5-HT4(a) (Fig.  6); 4) the above-mentioned inhibitors and dominant-negative constructs also effectively inhibited SRE activation induced by Galpha13; 5) finally, direct measurement of Rho activity using a rhotekin binding assay showed that the 5-HT4(a) receptor is able to activate Rho (Fig.  6 C).	bind
21370	5	6244	7	NULL	NULL	NULL	NULL	C3 exoenzyme	GP		inhibits					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_23_20812_s_295	11923294	1) Expression of wild type Galpha13 enhanced 5-HT4(a)-induced SRE activation (Fig.  5); 2) Galpha13 was inhibited by the RGS domain of p115RhoGEF, which is specific for Galpha12 and Galpha13 (Fig.  4); 3) C3 exoenzyme, a specific inhibitor of Rho proteins, inhibited SRE activation by 5-HT4(a) (Fig.  6); 4) the above-mentioned inhibitors and dominant-negative constructs also effectively inhibited SRE activation induced by Galpha13; 5) finally, direct measurement of Rho activity using a rhotekin binding assay showed that the 5-HT4(a) receptor is able to activate Rho (Fig.  6 C).	bind
21371	6	6244	7	NULL	NULL	NULL	NULL	C3 exoenzyme	GP		inhibits					Rho proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_23_20812_s_295	11923294	1) Expression of wild type Galpha13 enhanced 5-HT4(a)-induced SRE activation (Fig.  5); 2) Galpha13 was inhibited by the RGS domain of p115RhoGEF, which is specific for Galpha12 and Galpha13 (Fig.  4); 3) C3 exoenzyme, a specific inhibitor of Rho proteins, inhibited SRE activation by 5-HT4(a) (Fig.  6); 4) the above-mentioned inhibitors and dominant-negative constructs also effectively inhibited SRE activation induced by Galpha13; 5) finally, direct measurement of Rho activity using a rhotekin binding assay showed that the 5-HT4(a) receptor is able to activate Rho (Fig.  6 C).	bind
21376	7	6244	7	NULL	NULL	NULL	NULL	5-HT4 receptor	GP		activate					Rho	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_23_20812_s_295	11923294	1) Expression of wild type Galpha13 enhanced 5-HT4(a)-induced SRE activation (Fig.  5); 2) Galpha13 was inhibited by the RGS domain of p115RhoGEF, which is specific for Galpha12 and Galpha13 (Fig.  4); 3) C3 exoenzyme, a specific inhibitor of Rho proteins, inhibited SRE activation by 5-HT4(a) (Fig.  6); 4) the above-mentioned inhibitors and dominant-negative constructs also effectively inhibited SRE activation induced by Galpha13; 5) finally, direct measurement of Rho activity using a rhotekin binding assay showed that the 5-HT4(a) receptor is able to activate Rho (Fig.  6 C).	bind
55033	8	6244	7	NULL	NULL	NULL	NULL	 p115RhoGEF	GP		is specific for			RGS domain		Galpha12	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_23_20812_s_295	11923294	1) Expression of wild type Galpha13 enhanced 5-HT4(a)-induced SRE activation (Fig.  5); 2) Galpha13 was inhibited by the RGS domain of p115RhoGEF, which is specific for Galpha12 and Galpha13 (Fig.  4); 3) C3 exoenzyme, a specific inhibitor of Rho proteins, inhibited SRE activation by 5-HT4(a) (Fig.  6); 4) the above-mentioned inhibitors and dominant-negative constructs also effectively inhibited SRE activation induced by Galpha13; 5) finally, direct measurement of Rho activity using a rhotekin binding assay showed that the 5-HT4(a) receptor is able to activate Rho (Fig.  6 C).	bind
55035	9	6244	7	NULL	NULL	NULL	NULL	p115RhoGEF	GP		is specific for			RGS domain		Galpha13	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_23_20812_s_295	11923294	1) Expression of wild type Galpha13 enhanced 5-HT4(a)-induced SRE activation (Fig.  5); 2) Galpha13 was inhibited by the RGS domain of p115RhoGEF, which is specific for Galpha12 and Galpha13 (Fig.  4); 3) C3 exoenzyme, a specific inhibitor of Rho proteins, inhibited SRE activation by 5-HT4(a) (Fig.  6); 4) the above-mentioned inhibitors and dominant-negative constructs also effectively inhibited SRE activation induced by Galpha13; 5) finally, direct measurement of Rho activity using a rhotekin binding assay showed that the 5-HT4(a) receptor is able to activate Rho (Fig.  6 C).	bind
55036	10	6244	7	NULL	NULL	NULL	NULL	Galpha13	GP		induce							activation of		SRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_23_20812_s_295	11923294	1) Expression of wild type Galpha13 enhanced 5-HT4(a)-induced SRE activation (Fig.  5); 2) Galpha13 was inhibited by the RGS domain of p115RhoGEF, which is specific for Galpha12 and Galpha13 (Fig.  4); 3) C3 exoenzyme, a specific inhibitor of Rho proteins, inhibited SRE activation by 5-HT4(a) (Fig.  6); 4) the above-mentioned inhibitors and dominant-negative constructs also effectively inhibited SRE activation induced by Galpha13; 5) finally, direct measurement of Rho activity using a rhotekin binding assay showed that the 5-HT4(a) receptor is able to activate Rho (Fig.  6 C).	bind
55037	11	6244	7	NULL	NULL	NULL	NULL	p115RhoGEF	GP		inhibit		effectively			statement 10	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_23_20812_s_295	11923294	1) Expression of wild type Galpha13 enhanced 5-HT4(a)-induced SRE activation (Fig.  5); 2) Galpha13 was inhibited by the RGS domain of p115RhoGEF, which is specific for Galpha12 and Galpha13 (Fig.  4); 3) C3 exoenzyme, a specific inhibitor of Rho proteins, inhibited SRE activation by 5-HT4(a) (Fig.  6); 4) the above-mentioned inhibitors and dominant-negative constructs also effectively inhibited SRE activation induced by Galpha13; 5) finally, direct measurement of Rho activity using a rhotekin binding assay showed that the 5-HT4(a) receptor is able to activate Rho (Fig.  6 C).	bind
55039	12	6244	7	NULL	NULL	NULL	NULL	C3 exoenzyme	GP		inhibit		effectively			statement 10	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_23_20812_s_295	11923294	1) Expression of wild type Galpha13 enhanced 5-HT4(a)-induced SRE activation (Fig.  5); 2) Galpha13 was inhibited by the RGS domain of p115RhoGEF, which is specific for Galpha12 and Galpha13 (Fig.  4); 3) C3 exoenzyme, a specific inhibitor of Rho proteins, inhibited SRE activation by 5-HT4(a) (Fig.  6); 4) the above-mentioned inhibitors and dominant-negative constructs also effectively inhibited SRE activation induced by Galpha13; 5) finally, direct measurement of Rho activity using a rhotekin binding assay showed that the 5-HT4(a) receptor is able to activate Rho (Fig.  6 C).	bind
16803	1	6245	5	NULL	NULL	0	NULL	Gbeta	NULL		bind	NULL	specifically			CCT/TRiC complex	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_29_20221_s_330	16702223	1) Gbeta specifically binds CCT/TRiC (Figs.  5 and  6), a complex involved in protein folding ( ,  ,  ) and protein complex formation ( ,  ), shortly after its synthesis ( Fig. 8); there is a lag of several minutes before dimer formation, as would be expected if folding of Gbeta on CCT/TRiC is a requirement for production of functional Gbeta.	bind
16804	2	6245	5	NULL	NULL	0	NULL	CCT/TRiC complex	NULL		is involved in	NULL				protein folding	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_29_20221_s_330	16702223	1) Gbeta specifically binds CCT/TRiC (Figs.  5 and  6), a complex involved in protein folding ( ,  ,  ) and protein complex formation ( ,  ), shortly after its synthesis ( Fig. 8); there is a lag of several minutes before dimer formation, as would be expected if folding of Gbeta on CCT/TRiC is a requirement for production of functional Gbeta.	bind
16805	3	6245	5	NULL	NULL	0	NULL	CCT/TRiC complex	NULL		is involved in	NULL				protein complex formation, shortly after its synthesis	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_29_20221_s_330	16702223	1) Gbeta specifically binds CCT/TRiC (Figs.  5 and  6), a complex involved in protein folding ( ,  ,  ) and protein complex formation ( ,  ), shortly after its synthesis ( Fig. 8); there is a lag of several minutes before dimer formation, as would be expected if folding of Gbeta on CCT/TRiC is a requirement for production of functional Gbeta.	bind
21382	1	6245	7	NULL	NULL	NULL	NULL	Gbeta 	GP		binds		specifically			CCT/TRiC complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_29_20221_s_330	16702223	1) Gbeta specifically binds CCT/TRiC (Figs.  5 and  6), a complex involved in protein folding ( ,  ,  ) and protein complex formation ( ,  ), shortly after its synthesis ( Fig. 8); there is a lag of several minutes before dimer formation, as would be expected if folding of Gbeta on CCT/TRiC is a requirement for production of functional Gbeta.	bind
21386	2	6245	7	NULL	NULL	NULL	NULL	CCT/TRiC complex	GP		is involved in					protein folding	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_29_20221_s_330	16702223	1) Gbeta specifically binds CCT/TRiC (Figs.  5 and  6), a complex involved in protein folding ( ,  ,  ) and protein complex formation ( ,  ), shortly after its synthesis ( Fig. 8); there is a lag of several minutes before dimer formation, as would be expected if folding of Gbeta on CCT/TRiC is a requirement for production of functional Gbeta.	bind
21388	3	6245	7	NULL	NULL	NULL	NULL	CCT/TRiC complex	GP		is involved in					protein complex 	GP	formation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_29_20221_s_330	16702223	1) Gbeta specifically binds CCT/TRiC (Figs.  5 and  6), a complex involved in protein folding ( ,  ,  ) and protein complex formation ( ,  ), shortly after its synthesis ( Fig. 8); there is a lag of several minutes before dimer formation, as would be expected if folding of Gbeta on CCT/TRiC is a requirement for production of functional Gbeta.	bind
16806	1	6246	5	NULL	NULL	0	NULL	hyaluronan	NULL		bind	NULL				CD44	NULL	clustered			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_37_35111_s_377	11451952	1) hyaluronan binds to clustered CD44 and possibly other unknown cell surface receptors.	bind
16807	2	6246	5	NULL	NULL	0	NULL	hyaluronan	NULL		bind	NULL	possibly			cell surface receptors	NULL	other unknown			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_37_35111_s_377	11451952	1) hyaluronan binds to clustered CD44 and possibly other unknown cell surface receptors.	bind
21394	1	6246	7	NULL	NULL	NULL	NULL	hyaluronan	Chemical		binds					CD44	Cell	clustered 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_37_35111_s_377	11451952	1) hyaluronan binds to clustered CD44 and possibly other unknown cell surface receptors.	bind
21397	2	6246	7	NULL	NULL	NULL	NULL	hyaluronan	Chemical		binds		possibly			cell surface receptor	GP	unknown			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_37_35111_s_377	11451952	1) hyaluronan binds to clustered CD44 and possibly other unknown cell surface receptors.	bind
16809	1	6248	5	NULL	NULL	0	NULL	SopE2	NULL		bind	NULL				Rac1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_36_34035_s_197	11440999	1) In the absence of free guanine nucleotide, the equilibrium binding of SopE2 to Cdc42 is ~40-fold stronger than binding of SopE2 to Rac1.	bind
16810	2	6248	5	NULL	NULL	0	NULL	SopE2	NULL		bind	NULL				Cdc42	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_36_34035_s_197	11440999	1) In the absence of free guanine nucleotide, the equilibrium binding of SopE2 to Cdc42 is ~40-fold stronger than binding of SopE2 to Rac1.	bind
16811	3	6248	5	NULL	NULL	0	NULL	statement 2	NULL	equilibrium binding of 	is stronger than	NULL				statement 1	NULL	equilibrium binding of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_36_34035_s_197	11440999	1) In the absence of free guanine nucleotide, the equilibrium binding of SopE2 to Cdc42 is ~40-fold stronger than binding of SopE2 to Rac1.	bind
16812	4	6248	5	NULL	NULL	0	NULL	statement 3	NULL		in the absence of	NULL				guanine nucleotide	NULL	free			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_36_34035_s_197	11440999	1) In the absence of free guanine nucleotide, the equilibrium binding of SopE2 to Cdc42 is ~40-fold stronger than binding of SopE2 to Rac1.	bind
21403	1	6248	7	NULL	NULL	NULL	NULL	SopE2	GP		bind					Cdc42	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_36_34035_s_197	11440999	1) In the absence of free guanine nucleotide, the equilibrium binding of SopE2 to Cdc42 is ~40-fold stronger than binding of SopE2 to Rac1.	bind
21404	2	6248	7	NULL	NULL	NULL	NULL	SopE2	GP		bind					Rac1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_36_34035_s_197	11440999	1) In the absence of free guanine nucleotide, the equilibrium binding of SopE2 to Cdc42 is ~40-fold stronger than binding of SopE2 to Rac1.	bind
21408	3	6248	7	NULL	NULL	NULL	NULL	statement 1	Process	equilibrium binding of 	is stronger than					statement 2	Process	equilibrium binding of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_36_34035_s_197	11440999	1) In the absence of free guanine nucleotide, the equilibrium binding of SopE2 to Cdc42 is ~40-fold stronger than binding of SopE2 to Rac1.	bind
26360	4	6248	7	NULL	NULL	NULL	NULL	statement 3	Process		in the absence of					 guanine nucleotide	Chemical	free			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_36_34035_s_197	11440999	1) In the absence of free guanine nucleotide, the equilibrium binding of SopE2 to Cdc42 is ~40-fold stronger than binding of SopE2 to Rac1.	bind
16813	1	6250	5	NULL	NULL	0	NULL	pPL86 RNCs	NULL		bind	NULL				RM	NULL				NULL	translocation sites	0	NULL	NULL	NULL	gw60_jbiolchem_275_43_33828_s_247	10924518	1) In the study of Murphy  et al. ( 24), pPL86 RNCs were bound to RM in stoichiometric excess to translocation sites, and mild proteolysis was then performed to determine if a population of SRP receptor had become sequestered in a protease-resistant site.	bind
21414	1	6250	7	NULL	NULL	NULL	NULL	pPL86 RNCs	GP		bind					RM	CellComponent				NULL	translocation sites	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_43_33828_s_247	10924518	1) In the study of Murphy  et al. ( 24), pPL86 RNCs were bound to RM in stoichiometric excess to translocation sites, and mild proteolysis was then performed to determine if a population of SRP receptor had become sequestered in a protease-resistant site.	bind
16814	1	6251	5	NULL	NULL	0	NULL	FITC-Gal-PLL	NULL		bind	NULL				rML	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_27_16056_s_119	7541793	1) Ligand (FITC-Gal-PLL) binding to rML was not inhibited by LOM-11 ( Fig. 4).	bind
16815	2	6251	5	NULL	NULL	0	NULL	LOM-11	NULL		does not inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_27_16056_s_119	7541793	1) Ligand (FITC-Gal-PLL) binding to rML was not inhibited by LOM-11 ( Fig. 4).	bind
21416	1	6251	7	NULL	NULL	NULL	NULL	FITC-Gal-PLL	AminoAcid		bind					rML	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_27_16056_s_119	7541793	1) Ligand (FITC-Gal-PLL) binding to rML was not inhibited by LOM-11 ( Fig. 4).	bind
21417	2	6251	7	NULL	NULL	NULL	NULL	 LOM-11	GP		does not inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_27_16056_s_119	7541793	1) Ligand (FITC-Gal-PLL) binding to rML was not inhibited by LOM-11 ( Fig. 4).	bind
16816	1	6252	5	NULL	NULL	0	NULL	T3 	NULL		bind	NULL				TR	NULL				NULL	in solution	0	NULL	NULL	NULL	gw60_jbiolchem_273_46_30175_s_223	9804773	1) Most RTH mutations affect T3 binding to TR in solution or on DNA, as is the case with hinge mutants.	bind
16817	2	6252	5	NULL	NULL	0	NULL	T3	NULL		bind	NULL				TR	NULL				NULL	on DNA	0	NULL	NULL	NULL	gw60_jbiolchem_273_46_30175_s_223	9804773	1) Most RTH mutations affect T3 binding to TR in solution or on DNA, as is the case with hinge mutants.	bind
16818	3	6252	5	10	NULL	0	NULL	RTH 	NULL	mutation of	affect	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_46_30175_s_223	9804773	1) Most RTH mutations affect T3 binding to TR in solution or on DNA, as is the case with hinge mutants.	bind
16819	4	6252	5	10	NULL	0	NULL	RTH	NULL	mutation of	affect	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_46_30175_s_223	9804773	1) Most RTH mutations affect T3 binding to TR in solution or on DNA, as is the case with hinge mutants.	bind
16824	5	6252	5	NULL	NULL	0	NULL	hinge mutants	NULL		affect	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_46_30175_s_223	9804773	1) Most RTH mutations affect T3 binding to TR in solution or on DNA, as is the case with hinge mutants.	bind
16825	6	6252	5	NULL	NULL	0	NULL	hinge mutants	NULL		affect	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_46_30175_s_223	9804773	1) Most RTH mutations affect T3 binding to TR in solution or on DNA, as is the case with hinge mutants.	bind
21418	1	6252	7	NULL	NULL	NULL	NULL	T3	GP		bind					TR	GP				NULL	in solution	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_46_30175_s_223	9804773	1) Most RTH mutations affect T3 binding to TR in solution or on DNA, as is the case with hinge mutants.	bind
21420	2	6252	7	NULL	NULL	NULL	NULL	T3	GP		bind					TR	GP				NULL	on DNA	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_46_30175_s_223	9804773	1) Most RTH mutations affect T3 binding to TR in solution or on DNA, as is the case with hinge mutants.	bind
21423	3	6252	7	NULL	NULL	NULL	NULL	RTH	Process	mutation of	affect					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_46_30175_s_223	9804773	1) Most RTH mutations affect T3 binding to TR in solution or on DNA, as is the case with hinge mutants.	bind
21428	4	6252	7	NULL	NULL	NULL	NULL	RTH	Process	mutation of	affect					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_46_30175_s_223	9804773	1) Most RTH mutations affect T3 binding to TR in solution or on DNA, as is the case with hinge mutants.	bind
26362	5	6252	7	NULL	NULL	NULL	NULL	hinge mutants	Chemical		affect					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_46_30175_s_223	9804773	1) Most RTH mutations affect T3 binding to TR in solution or on DNA, as is the case with hinge mutants.	bind
26363	6	6252	7	NULL	NULL	NULL	NULL	hinge mutants	Chemical		affect					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_46_30175_s_223	9804773	1) Most RTH mutations affect T3 binding to TR in solution or on DNA, as is the case with hinge mutants.	bind
16828	1	6253	5	NULL	NULL	0	NULL	HSPG	NULL		is	NULL				heparan sulfate proteoglycans	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16829	2	6253	5	NULL	NULL	0	NULL	MV	NULL		is	NULL				microvilli	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16830	3	6253	5	NULL	NULL	0	NULL	HSPG	NULL		is distributed on	NULL	mostly			MV	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16833	4	6253	5	NULL	NULL	0	NULL	LPL	NULL		bind	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16835	5	6253	5	NULL	NULL	0	NULL	LPL-TRL	NULL		bind	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16836	6	6253	5	NULL	NULL	0	NULL	nCV	NULL		is	NULL				non-coated pit vesicles	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16838	7	6253	5	NULL	NULL	0	NULL	LPL & associated TRL	NULL		is internalized by	NULL				HSPG	NULL				NULL	in nCV	0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16843	8	6253	5	NULL	NULL	0	NULL	nCV	NULL	after uptake	meet	NULL				EE	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16844	9	6253	5	NULL	NULL	0	NULL	EE	NULL		is	NULL				early endosomes	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16845	10	6253	5	NULL	NULL	0	NULL	nCV	NULL	after uptake	fuse to	NULL				EE	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16846	11	6253	5	NULL	NULL	0	NULL	statement 10	NULL		is an alternative to	NULL				statement 8	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16847	12	6253	5	NULL	NULL	0	NULL	LPL	NULL		seperate from	NULL				TRL	NULL				NULL	in EE	0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16848	13	6253	5	NULL	NULL	0	NULL	LPL	NULL		is delivered to	NULL				MVB	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16849	14	6253	5	NULL	NULL	0	NULL	MVB	NULL		is	NULL				multivesicular bodies	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16850	15	6253	5	NULL	NULL	0	NULL	LPL	NULL		is delivered to	NULL	probably			Lys	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16851	16	6253	5	NULL	NULL	0	NULL	Lys	NULL		is	NULL				lysosomes	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16852	17	6253	5	NULL	NULL	0	NULL	TRL	NULL		is retained within	NULL				EE	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16853	18	6253	5	NULL	NULL	0	NULL	TRL	NULL		is retained within	NULL				compartments	NULL	other			NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16854	19	6253	5	NULL	NULL	0	NULL	statement 17	NULL		is an alternative to	NULL				statement 18	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16855	20	6253	5	NULL	NULL	0	NULL	LPL	NULL	some	bind	NULL				HSPG	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16856	21	6253	5	NULL	NULL	0	NULL	TRL	NULL	some LPL-associated	bind	NULL				HSPG	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16857	22	6253	5	NULL	NULL	0	NULL	statement 20	NULL		recognized by	NULL	could be			LRP	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16858	23	6253	5	NULL	NULL	0	NULL	statement 21	NULL		recognized by	NULL	could be			LDLr	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16859	24	6253	5	NULL	NULL	0	NULL	statement 22	NULL		is an alternative to	NULL				statement 23	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16860	25	6253	5	NULL	NULL	0	NULL	statement 20	NULL		taken up by	NULL	could be			LRP	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16861	26	6253	5	NULL	NULL	0	NULL	statement 21	NULL		taken up by	NULL	could be			LDLr	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16862	27	6253	5	NULL	NULL	0	NULL	statement 25	NULL		is an alternative to	NULL				statement 26	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16863	28	6253	5	NULL	NULL	0	NULL	cv	NULL		is	NULL				coated pit	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16864	29	6253	5	NULL	NULL	0	NULL	statement 25	NULL		follows	NULL				cv endocytosis pathway	NULL	to lysosomes			NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16865	30	6253	5	NULL	NULL	0	NULL	statement 26	NULL		follows	NULL				cv endocytosis pathway	NULL	to lysosomes			NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16866	31	6253	5	NULL	NULL	0	NULL	TRL	NULL		is recognized by	NULL				coated pit-associated receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16867	32	6253	5	NULL	NULL	0	NULL	TRL	NULL		is internalized by	NULL				coated pit-associated receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16868	33	6253	5	NULL	NULL	0	NULL	statement 31	NULL		in the absence of	NULL				LPL	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
16869	34	6253	5	NULL	NULL	0	NULL	statement 32	NULL		in the absence of	NULL				LPL	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
21491	1	6253	7	NULL	NULL	NULL	NULL	LPL	GP		are distributed in			Primary binding-site		HSPG	Chemical	microvilli 			NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
21492	2	6253	7	NULL	NULL	NULL	NULL	LPL-TRL	GP		are distributed in			Primary binding-site		HSPG	Chemical	microvilli 			NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
21493	3	6253	7	NULL	NULL	NULL	NULL	 LPL	GP		associate with					TRL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
21494	4	6253	7	NULL	NULL	NULL	NULL	statement 3	Process		is internalized					HSPG	Chemical	in nCV			NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
21495	5	6253	7	NULL	NULL	NULL	NULL	nCV	CellComponent		fuse to					EE	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
21496	6	6253	7	NULL	NULL	NULL	NULL	LPL	GP		separate from					TRL	GP				NULL	in EE	NULL	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
21497	7	6253	7	NULL	NULL	NULL	NULL	LPL	GP		delivered to					MVB	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
21498	8	6253	7	NULL	NULL	NULL	NULL	LPL	GP		delivered to					Lys	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
21499	9	6253	7	NULL	NULL	NULL	NULL	TRL	GP		is retained within					early endosomes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
21500	10	6253	7	NULL	NULL	NULL	NULL	LPL	GP		bind					HSPG	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
21501	11	6253	7	NULL	NULL	NULL	NULL	TRL	GP	LPL-associated	bind					HSPG	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
21502	12	6253	7	NULL	NULL	NULL	NULL	statement 10	Process		taken up by					LRP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
21503	13	6253	7	NULL	NULL	NULL	NULL	statement 11	Process		taken up by					LRP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
21504	14	6253	7	NULL	NULL	NULL	NULL	statement 10	Process		taken up by					LDLr	GP				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
21505	15	6253	7	NULL	NULL	NULL	NULL	statement 11	Process		taken up by					LDLr	GP				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
21506	16	6253	7	NULL	NULL	NULL	NULL	statement 14	Process		is an alternative to					statement 12	Process				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
21507	17	6253	7	NULL	NULL	NULL	NULL	statement 15	Process		is an alternative to					statement 13	Process				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
21508	18	6253	7	NULL	NULL	NULL	NULL	statement 12	Process		follows to					coated pit endocytosis pathway to the lysosomes	Process				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
21509	19	6253	7	NULL	NULL	NULL	NULL	statement 13	Process		follows to					coated pit endocytosis pathway to the lysosomes	Process				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
21510	20	6253	7	NULL	NULL	NULL	NULL	statement 14	Process		follows to					coated pit endocytosis pathway to the lysosomes	Process				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
21511	21	6253	7	NULL	NULL	NULL	NULL	statement 15	Process		follows to					coated pit endocytosis pathway to the lysosomes	Process				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
21512	22	6253	7	NULL	NULL	NULL	NULL	 TRL 	GP		is internalized by					coated pit-associated receptors	Process				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
21513	23	6253	7	NULL	NULL	NULL	NULL	statement 22	Process		occurs in absence of					LPL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
21514	24	6253	7	NULL	NULL	NULL	NULL	HSPG	Chemical		is					heparan sulfate proteoglycans	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
21515	25	6253	7	NULL	NULL	NULL	NULL	MV	OrganismPart		is					microvilli	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
21516	26	6253	7	NULL	NULL	NULL	NULL	nCV	CellComponent		is					non-coated pit vesicles	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
21517	27	6253	7	NULL	NULL	NULL	NULL	EE	CellComponent		is					early endosomes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
21518	28	6253	7	NULL	NULL	NULL	NULL	MVB	CellComponent		is					multivesicular bodies	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
21519	29	6253	7	NULL	NULL	NULL	NULL	Lys	CellComponent		is					lysosomes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
21520	30	6253	7	NULL	NULL	NULL	NULL	cv	CellComponent		is					 coated pit	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_39_4_789_s_317	9555944	1) Primary binding-sites for LPL and LPL-TRL are heparan sulfate proteoglycans (HSPG), which are distributed mostly on the microvilli (MV); 2) LPL together with associated TRL are internalized by HSPG in non-coated pit vesicles (nCV); 3) after uptake, these vesicles meet or fuse to early endosomes (EE), where LPL and TRL could separate; 4) LPL is delivered to multivesicular bodies (MVB) and probably to lysosomes (Lys); 5) TRL are retained either within the same early endosomes or in other compartments; 6) alternatively, some LPL and LPL-associated TRL bound to HSPG could be recognized and taken up by LRP or by LDLr following the coated pit (cv) endocytosis pathway to the lysosomes; 7) in the absence of LPL, TRL are recognized and internalized by coated pit-associated receptors.	bind
19264	1	6254	5	NULL	NULL	0	NULL	Rab family members	NULL		bind	NULL				GDP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
19265	2	6254	5	NULL	NULL	0	NULL	Rab GDI	NULL		bind	NULL	preferentially			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
19266	4	6254	5	NULL	NULL	0	NULL	statement 1	NULL		is converted to	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
19267	5	6254	5	NULL	NULL	0	NULL	Rab GEP	NULL	action of each	is required for	NULL				statement 4	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
19268	6	6254	5	NULL	NULL	0	NULL	Rab GDI	NULL		prevents	NULL				statement 4	NULL				NULL	in cytosol	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
19269	7	6254	5	NULL	NULL	0	NULL	Rab family members	NULL		is kept as	NULL				statement 1	NULL				NULL	in cytosol	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
19270	8	6254	5	NULL	NULL	0	NULL	statement 6	NULL		results in	NULL				statement 7	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
19271	9	6254	5	NULL	NULL	0	NULL	Rab GDI	NULL		is associated with	NULL				target membranes	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
19272	10	6254	5	NULL	NULL	0	NULL	statement 9	NULL		results in	NULL				statement 7	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
19273	11	6254	5	NULL	NULL	0	NULL	Rab family members	NULL	complexed	is transported to	NULL				target membranes	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
19274	13	6254	5	NULL	NULL	0	NULL	statement 1	NULL		is dissociated from	NULL				Rab GDI	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
19275	14	6254	5	NULL	NULL	0	NULL	statement 11	NULL		leads to	NULL				statement 13	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
19276	15	6254	5	NULL	NULL	0	NULL	Rab GDI displacement factor	NULL	action of each putative	is required for	NULL				statement 13	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
19277	16	6254	5	NULL	NULL	0	NULL	statement 15	NULL		is followed by	NULL				statement 4	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
19278	17	6254	5	NULL	NULL	0	NULL	statement 3	NULL		is converted to	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
19279	18	6254	5	NULL	NULL	0	NULL	Rab GAP	NULL	action of each	is required for	NULL				statement 17	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
46191	3	6254	5	NULL	NULL	0	NULL	Rab family members	NULL		bind	NULL				GTP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
46193	12	6254	5	NULL	NULL	0	NULL	Rab GDI	NULL		is required for	NULL				statement 11	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
21521	2	6254	7	NULL	NULL	NULL	NULL	Rab GDI	GP		interacts with		preferentially			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
21522	3	6254	7	NULL	NULL	NULL	NULL	statement 2	Process		keeps					statement 1	Process				NULL	in the cytosol	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
21523	5	6254	7	NULL	NULL	NULL	NULL	statement 1	Process		converts to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
21524	6	6254	7	NULL	NULL	NULL	NULL	statement 5	Process		is converted by					Rab GEP 	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
21525	7	6254	7	NULL	NULL	NULL	NULL	statement 3	Process		prevents					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
21526	8	6254	7	NULL	NULL	NULL	NULL	statement 1	Process		associate with					target membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
21529	11	6254	7	NULL	NULL	NULL	NULL	Rab GDI displacement factor	GP	 putative	dissociates					statement 2	Process	GDP from			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
21530	12	6254	7	NULL	NULL	NULL	NULL	statement 11	Process		is followed by					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
45637	1	6254	7	NULL	NULL	NULL	NULL	GDP	Chemical		bind					Rab family members	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
45638	4	6254	7	NULL	NULL	NULL	NULL	GTP	Chemical		bind					Rab family members	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
45639	9	6254	7	NULL	NULL	NULL	NULL	statement 3	Process		prevents					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
45640	10	6254	7	NULL	NULL	NULL	NULL	Rab GDI	GP		transports					statement 2	Process	to target membranes			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
45641	13	6254	7	NULL	NULL	NULL	NULL	statement 4	Process		accomplishes					function	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
45642	14	6254	7	NULL	NULL	NULL	NULL	statement 13	Process		is converted to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
45643	15	6254	7	NULL	NULL	NULL	NULL	Rab GAP	GP		converts					statement 14	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34580_s_26	9852129	1) Rab GDI preferentially interacts with the GDP-bound form of Rab family members and keeps them in the GDP-bound form in the cytosol by preventing them from being converted to the GTP-bound form by the action of each Rab GEP and from being associated with each of their target membranes; 2) Rab GDI transports its complexed Rab family members to each of their target membranes where the GDP-bound form dissociates from Rab GDI by the action of each putative Rab GDI displacement factor, followed by conversion to the GTP-bound form by the action of each Rab GEP; and 3) after the GTP-bound form accomplishes its function, it is converted to the GDP-bound form by the action of each Rab GAP.	bind
16870	1	6255	5	NULL	NULL	0	NULL	RAP74	NULL		bind	NULL				TFIIB	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_20_11703_s_206	8662660	1) RAP74 could bind TFIIB to block the RAP30 binding site  on TFIIB.	bind
16871	2	6255	5	NULL	NULL	0	NULL	statement 1	NULL		block	NULL				TFIIB	NULL		RAP30 binding site		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_20_11703_s_206	8662660	1) RAP74 could bind TFIIB to block the RAP30 binding site  on TFIIB.	bind
21534	1	6255	7	NULL	NULL	NULL	NULL	RAP74	GP		bind					TFIIB	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_20_11703_s_206	8662660	1) RAP74 could bind TFIIB to block the RAP30 binding site  on TFIIB.	bind
21535	2	6255	7	NULL	NULL	NULL	NULL	statement 1	Process		blocks					TFIIB	GP		RAP30 binding site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_20_11703_s_206	8662660	1) RAP74 could bind TFIIB to block the RAP30 binding site  on TFIIB.	bind
16872	1	6256	5	NULL	NULL	0	NULL	TR homodimers	NULL		bind	NULL					NULL	positive		TREs	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_24_14274_s_85	7782283	1) T   binding  dissociates TR homodimers from positive TREs ( 39) (see  Fig. 7 A), allowing preferential binding of TR RXR  heterodimers; 2) TR RXR heterodimers have a stronger affinity for  TREs than TR homodimers( 8) ; 3) cotransfection of RXR enhances  the positive transcriptional response to T   on a number of  different elements( 10,  40) ; and 4) more recently yeast  expression systems demonstrate that TR RXR heterodimerization is  necessary for a full ligand-dependent transcriptional  response( 41) .	bind
16873	2	6256	5	NULL	NULL	0	NULL	T binding	NULL		dissociates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_24_14274_s_85	7782283	1) T   binding  dissociates TR homodimers from positive TREs ( 39) (see  Fig. 7 A), allowing preferential binding of TR RXR  heterodimers; 2) TR RXR heterodimers have a stronger affinity for  TREs than TR homodimers( 8) ; 3) cotransfection of RXR enhances  the positive transcriptional response to T   on a number of  different elements( 10,  40) ; and 4) more recently yeast  expression systems demonstrate that TR RXR heterodimerization is  necessary for a full ligand-dependent transcriptional  response( 41) .	bind
16874	3	6256	5	NULL	NULL	0	NULL	statement 2	NULL		allows	NULL				TR RXR heterodimers	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_24_14274_s_85	7782283	1) T   binding  dissociates TR homodimers from positive TREs ( 39) (see  Fig. 7 A), allowing preferential binding of TR RXR  heterodimers; 2) TR RXR heterodimers have a stronger affinity for  TREs than TR homodimers( 8) ; 3) cotransfection of RXR enhances  the positive transcriptional response to T   on a number of  different elements( 10,  40) ; and 4) more recently yeast  expression systems demonstrate that TR RXR heterodimerization is  necessary for a full ligand-dependent transcriptional  response( 41) .	bind
16875	4	6256	5	NULL	NULL	0	NULL	TR RXR heterodimers	NULL		bind	NULL					NULL			TREs	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_24_14274_s_85	7782283	1) T   binding  dissociates TR homodimers from positive TREs ( 39) (see  Fig. 7 A), allowing preferential binding of TR RXR  heterodimers; 2) TR RXR heterodimers have a stronger affinity for  TREs than TR homodimers( 8) ; 3) cotransfection of RXR enhances  the positive transcriptional response to T   on a number of  different elements( 10,  40) ; and 4) more recently yeast  expression systems demonstrate that TR RXR heterodimerization is  necessary for a full ligand-dependent transcriptional  response( 41) .	bind
16876	5	6256	5	NULL	NULL	0	NULL	TR RXR heterodimers	NULL		bind	NULL				TR homodimers	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_24_14274_s_85	7782283	1) T   binding  dissociates TR homodimers from positive TREs ( 39) (see  Fig. 7 A), allowing preferential binding of TR RXR  heterodimers; 2) TR RXR heterodimers have a stronger affinity for  TREs than TR homodimers( 8) ; 3) cotransfection of RXR enhances  the positive transcriptional response to T   on a number of  different elements( 10,  40) ; and 4) more recently yeast  expression systems demonstrate that TR RXR heterodimerization is  necessary for a full ligand-dependent transcriptional  response( 41) .	bind
16877	6	6256	5	NULL	NULL	0	NULL	statement 4	NULL		stronger affinity than	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_24_14274_s_85	7782283	1) T   binding  dissociates TR homodimers from positive TREs ( 39) (see  Fig. 7 A), allowing preferential binding of TR RXR  heterodimers; 2) TR RXR heterodimers have a stronger affinity for  TREs than TR homodimers( 8) ; 3) cotransfection of RXR enhances  the positive transcriptional response to T   on a number of  different elements( 10,  40) ; and 4) more recently yeast  expression systems demonstrate that TR RXR heterodimerization is  necessary for a full ligand-dependent transcriptional  response( 41) .	bind
16878	7	6256	5	10	NULL	0	NULL	RXR		cotransfection of 	enhance					T		positive transcriptional response to			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_24_14274_s_85	7782283	1) T   binding  dissociates TR homodimers from positive TREs ( 39) (see  Fig. 7 A), allowing preferential binding of TR RXR  heterodimers; 2) TR RXR heterodimers have a stronger affinity for  TREs than TR homodimers( 8) ; 3) cotransfection of RXR enhances  the positive transcriptional response to T   on a number of  different elements( 10,  40) ; and 4) more recently yeast  expression systems demonstrate that TR RXR heterodimerization is  necessary for a full ligand-dependent transcriptional  response( 41) .	bind
16879	8	6256	5	10	NULL	0	NULL	TR RXR		heterodimerization of	is necessary for					statement 9					NULL	yeast expression systems	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_24_14274_s_85	7782283	1) T   binding  dissociates TR homodimers from positive TREs ( 39) (see  Fig. 7 A), allowing preferential binding of TR RXR  heterodimers; 2) TR RXR heterodimers have a stronger affinity for  TREs than TR homodimers( 8) ; 3) cotransfection of RXR enhances  the positive transcriptional response to T   on a number of  different elements( 10,  40) ; and 4) more recently yeast  expression systems demonstrate that TR RXR heterodimerization is  necessary for a full ligand-dependent transcriptional  response( 41) .	bind
54174	9	6256	5	10	NULL	0	NULL	transcriptional response			is dependent on		fully			ligand					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_24_14274_s_85	7782283	1) T   binding  dissociates TR homodimers from positive TREs ( 39) (see  Fig. 7 A), allowing preferential binding of TR RXR  heterodimers; 2) TR RXR heterodimers have a stronger affinity for  TREs than TR homodimers( 8) ; 3) cotransfection of RXR enhances  the positive transcriptional response to T   on a number of  different elements( 10,  40) ; and 4) more recently yeast  expression systems demonstrate that TR RXR heterodimerization is  necessary for a full ligand-dependent transcriptional  response( 41) .	bind
21536	1	6256	7	NULL	NULL	NULL	NULL	TR homodimers	GP		dissociates from							positive		TREs	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_24_14274_s_85	7782283	1) T   binding  dissociates TR homodimers from positive TREs ( 39) (see  Fig. 7 A), allowing preferential binding of TR RXR  heterodimers; 2) TR RXR heterodimers have a stronger affinity for  TREs than TR homodimers( 8) ; 3) cotransfection of RXR enhances  the positive transcriptional response to T   on a number of  different elements( 10,  40) ; and 4) more recently yeast  expression systems demonstrate that TR RXR heterodimerization is  necessary for a full ligand-dependent transcriptional  response( 41) .	bind
21537	2	6256	7	NULL	NULL	NULL	NULL	T	Chemical	binding of	allows					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_24_14274_s_85	7782283	1) T   binding  dissociates TR homodimers from positive TREs ( 39) (see  Fig. 7 A), allowing preferential binding of TR RXR  heterodimers; 2) TR RXR heterodimers have a stronger affinity for  TREs than TR homodimers( 8) ; 3) cotransfection of RXR enhances  the positive transcriptional response to T   on a number of  different elements( 10,  40) ; and 4) more recently yeast  expression systems demonstrate that TR RXR heterodimerization is  necessary for a full ligand-dependent transcriptional  response( 41) .	bind
21538	3	6256	7	NULL	NULL	NULL	NULL	statement 2	Process		allows		preferentially			TR RXR heterodimers	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_24_14274_s_85	7782283	1) T   binding  dissociates TR homodimers from positive TREs ( 39) (see  Fig. 7 A), allowing preferential binding of TR RXR  heterodimers; 2) TR RXR heterodimers have a stronger affinity for  TREs than TR homodimers( 8) ; 3) cotransfection of RXR enhances  the positive transcriptional response to T   on a number of  different elements( 10,  40) ; and 4) more recently yeast  expression systems demonstrate that TR RXR heterodimerization is  necessary for a full ligand-dependent transcriptional  response( 41) .	bind
21539	4	6256	7	NULL	NULL	NULL	NULL	TR RXR heterodimers	GP		 affinity for		stronger							TRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_24_14274_s_85	7782283	1) T   binding  dissociates TR homodimers from positive TREs ( 39) (see  Fig. 7 A), allowing preferential binding of TR RXR  heterodimers; 2) TR RXR heterodimers have a stronger affinity for  TREs than TR homodimers( 8) ; 3) cotransfection of RXR enhances  the positive transcriptional response to T   on a number of  different elements( 10,  40) ; and 4) more recently yeast  expression systems demonstrate that TR RXR heterodimerization is  necessary for a full ligand-dependent transcriptional  response( 41) .	bind
21540	5	6256	7	NULL	NULL	NULL	NULL	TR homodimers	GP		has affinity for									TRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_24_14274_s_85	7782283	1) T   binding  dissociates TR homodimers from positive TREs ( 39) (see  Fig. 7 A), allowing preferential binding of TR RXR  heterodimers; 2) TR RXR heterodimers have a stronger affinity for  TREs than TR homodimers( 8) ; 3) cotransfection of RXR enhances  the positive transcriptional response to T   on a number of  different elements( 10,  40) ; and 4) more recently yeast  expression systems demonstrate that TR RXR heterodimerization is  necessary for a full ligand-dependent transcriptional  response( 41) .	bind
21541	6	6256	7	NULL	NULL	NULL	NULL	statement 4	Process		is stronger than					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_24_14274_s_85	7782283	1) T   binding  dissociates TR homodimers from positive TREs ( 39) (see  Fig. 7 A), allowing preferential binding of TR RXR  heterodimers; 2) TR RXR heterodimers have a stronger affinity for  TREs than TR homodimers( 8) ; 3) cotransfection of RXR enhances  the positive transcriptional response to T   on a number of  different elements( 10,  40) ; and 4) more recently yeast  expression systems demonstrate that TR RXR heterodimerization is  necessary for a full ligand-dependent transcriptional  response( 41) .	bind
21542	7	6256	7	NULL	NULL	NULL	NULL	RXR	GP	cotransfection of	enhances					T	Chemical	positive transcriptional response to			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_24_14274_s_85	7782283	1) T   binding  dissociates TR homodimers from positive TREs ( 39) (see  Fig. 7 A), allowing preferential binding of TR RXR  heterodimers; 2) TR RXR heterodimers have a stronger affinity for  TREs than TR homodimers( 8) ; 3) cotransfection of RXR enhances  the positive transcriptional response to T   on a number of  different elements( 10,  40) ; and 4) more recently yeast  expression systems demonstrate that TR RXR heterodimerization is  necessary for a full ligand-dependent transcriptional  response( 41) .	bind
21543	8	6256	7	NULL	NULL	NULL	NULL	TR RXR	GP	heterodimerization of	is necessary for					statement 9	Process				NULL	yeast expression systems	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_24_14274_s_85	7782283	1) T   binding  dissociates TR homodimers from positive TREs ( 39) (see  Fig. 7 A), allowing preferential binding of TR RXR  heterodimers; 2) TR RXR heterodimers have a stronger affinity for  TREs than TR homodimers( 8) ; 3) cotransfection of RXR enhances  the positive transcriptional response to T   on a number of  different elements( 10,  40) ; and 4) more recently yeast  expression systems demonstrate that TR RXR heterodimerization is  necessary for a full ligand-dependent transcriptional  response( 41) .	bind
54175	9	6256	7	NULL	NULL	NULL	NULL	transcriptional response	Process		is dependent on		fully			ligand	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_24_14274_s_85	7782283	1) T   binding  dissociates TR homodimers from positive TREs ( 39) (see  Fig. 7 A), allowing preferential binding of TR RXR  heterodimers; 2) TR RXR heterodimers have a stronger affinity for  TREs than TR homodimers( 8) ; 3) cotransfection of RXR enhances  the positive transcriptional response to T   on a number of  different elements( 10,  40) ; and 4) more recently yeast  expression systems demonstrate that TR RXR heterodimerization is  necessary for a full ligand-dependent transcriptional  response( 41) .	bind
16880	1	6257	5	NULL	NULL	0	NULL	IL-6	NULL		bind	NULL				M1-UR21 cells	NULL	nontransfected			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_35_22701_s_185	9712900	1) The affinity of IL-6 binding to nontransfected M1-UR21 cells, which express only low affinity receptors (IL-6R), was too low for an accurate estimation of the  K D.	bind
26374	1	6257	7	NULL	NULL	NULL	NULL	IL-6	GP		bind					M1-UR21 cells	Cell	 nontransfected			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_35_22701_s_185	9712900	1) The affinity of IL-6 binding to nontransfected M1-UR21 cells, which express only low affinity receptors (IL-6R), was too low for an accurate estimation of the  K D.	bind
16881	1	6258	5	NULL	NULL	0	NULL	glucitol	NULL		bind	NULL				GutR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_13_9620_s_274	11118449	1) The binding of glucitol to GutR can induce GutR to have conformational changes so that more residues in the DNA binding region of GutR are available to make extensive contacts with the GutR binding site.	bind
16882	2	6258	5	NULL	NULL	0	NULL	statement 1	NULL		induce	NULL				GutR	NULL	conformational changes in			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_13_9620_s_274	11118449	1) The binding of glucitol to GutR can induce GutR to have conformational changes so that more residues in the DNA binding region of GutR are available to make extensive contacts with the GutR binding site.	bind
21546	1	6258	7	NULL	NULL	NULL	NULL	glucitol 	Chemical		bind					GutR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_13_9620_s_274	11118449	1) The binding of glucitol to GutR can induce GutR to have conformational changes so that more residues in the DNA binding region of GutR are available to make extensive contacts with the GutR binding site.	bind
21547	2	6258	7	NULL	NULL	NULL	NULL	statement 1	Process		induce					GutR	GP	availability of	 DNA binding region of 		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_13_9620_s_274	11118449	1) The binding of glucitol to GutR can induce GutR to have conformational changes so that more residues in the DNA binding region of GutR are available to make extensive contacts with the GutR binding site.	bind
21548	3	6258	7	NULL	NULL	NULL	NULL	statement 2	Process		allows							extensive contacts with 	GutR binding site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_13_9620_s_274	11118449	1) The binding of glucitol to GutR can induce GutR to have conformational changes so that more residues in the DNA binding region of GutR are available to make extensive contacts with the GutR binding site.	bind
16883	1	6259	5	NULL	NULL	0	NULL	natriuretic peptide	NULL		bind	NULL					NULL		ECD		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_14_9752_s_28	10092664	1) The binding of the natriuretic peptide to ECD induces a conformational change.	bind
16884	2	6259	5	NULL	NULL	0	NULL	statement 1	NULL		induce	NULL					NULL	conformational change of	ECD		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_14_9752_s_28	10092664	1) The binding of the natriuretic peptide to ECD induces a conformational change.	bind
21549	1	6259	7	NULL	NULL	NULL	NULL	natriuretic peptide	GP		binds								ECD		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_14_9752_s_28	10092664	1) The binding of the natriuretic peptide to ECD induces a conformational change.	bind
21550	2	6259	7	NULL	NULL	NULL	NULL	statement 1	Process		induce							conformational change	ECD		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_14_9752_s_28	10092664	1) The binding of the natriuretic peptide to ECD induces a conformational change.	bind
16885	1	6260	5	NULL	NULL	0	NULL	PARP-1 inhibitors	NULL		decrease	NULL				AM-PARP	NULL	amounts of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_41_42774_s_401	15302869	1) The inhibitors of PARP-1 and the antisense RNA for PARP-1 mRNA decreased the amounts of AM-PARP and the expression of TNF-alpha and iNOS (Figs.  1,  2,  3) and the LPS-induced DNA binding of NF-kappaB ( Fig. 5).	bind
16886	2	6260	5	NULL	NULL	0	NULL	PARP-1 inhibitors	NULL		decrease	NULL				TNF-alpha	NULL	expression of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_41_42774_s_401	15302869	1) The inhibitors of PARP-1 and the antisense RNA for PARP-1 mRNA decreased the amounts of AM-PARP and the expression of TNF-alpha and iNOS (Figs.  1,  2,  3) and the LPS-induced DNA binding of NF-kappaB ( Fig. 5).	bind
16887	3	6260	5	NULL	NULL	0	NULL	PARP-1 inhibitors	NULL		decrease	NULL				iNOS	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_41_42774_s_401	15302869	1) The inhibitors of PARP-1 and the antisense RNA for PARP-1 mRNA decreased the amounts of AM-PARP and the expression of TNF-alpha and iNOS (Figs.  1,  2,  3) and the LPS-induced DNA binding of NF-kappaB ( Fig. 5).	bind
16888	4	6260	5	NULL	NULL	0	NULL	NF-kappaB	NULL		bind	NULL				DNA	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_41_42774_s_401	15302869	1) The inhibitors of PARP-1 and the antisense RNA for PARP-1 mRNA decreased the amounts of AM-PARP and the expression of TNF-alpha and iNOS (Figs.  1,  2,  3) and the LPS-induced DNA binding of NF-kappaB ( Fig. 5).	bind
16889	5	6260	5	NULL	NULL	0	NULL	LPS	NULL		induce	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_41_42774_s_401	15302869	1) The inhibitors of PARP-1 and the antisense RNA for PARP-1 mRNA decreased the amounts of AM-PARP and the expression of TNF-alpha and iNOS (Figs.  1,  2,  3) and the LPS-induced DNA binding of NF-kappaB ( Fig. 5).	bind
16890	6	6260	5	NULL	NULL	0	NULL	PARP-1 inhibitors	NULL		decrease	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_41_42774_s_401	15302869	1) The inhibitors of PARP-1 and the antisense RNA for PARP-1 mRNA decreased the amounts of AM-PARP and the expression of TNF-alpha and iNOS (Figs.  1,  2,  3) and the LPS-induced DNA binding of NF-kappaB ( Fig. 5).	bind
16891	7	6260	5	NULL	NULL	0	NULL	PARP-1 mRNA	NULL	antisense	decrease	NULL				AM-PARP	NULL	amounts of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_41_42774_s_401	15302869	1) The inhibitors of PARP-1 and the antisense RNA for PARP-1 mRNA decreased the amounts of AM-PARP and the expression of TNF-alpha and iNOS (Figs.  1,  2,  3) and the LPS-induced DNA binding of NF-kappaB ( Fig. 5).	bind
16892	8	6260	5	NULL	NULL	0	NULL	PARP-1 mRNA	NULL	antisense	decrease	NULL				TNF-alpha	NULL	expression of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_41_42774_s_401	15302869	1) The inhibitors of PARP-1 and the antisense RNA for PARP-1 mRNA decreased the amounts of AM-PARP and the expression of TNF-alpha and iNOS (Figs.  1,  2,  3) and the LPS-induced DNA binding of NF-kappaB ( Fig. 5).	bind
16893	9	6260	5	NULL	NULL	0	NULL	PARP-1 mRNA	NULL	antisense	decrease	NULL				iNOS	NULL	expression of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_41_42774_s_401	15302869	1) The inhibitors of PARP-1 and the antisense RNA for PARP-1 mRNA decreased the amounts of AM-PARP and the expression of TNF-alpha and iNOS (Figs.  1,  2,  3) and the LPS-induced DNA binding of NF-kappaB ( Fig. 5).	bind
16894	10	6260	5	NULL	NULL	0	NULL	PARP-1 mRNA	NULL	antisense	decrease	NULL				statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_41_42774_s_401	15302869	1) The inhibitors of PARP-1 and the antisense RNA for PARP-1 mRNA decreased the amounts of AM-PARP and the expression of TNF-alpha and iNOS (Figs.  1,  2,  3) and the LPS-induced DNA binding of NF-kappaB ( Fig. 5).	bind
21580	1	6260	7	NULL	NULL	NULL	NULL	PARP-1 inhibitor	Chemical		decrease					AM-PARP	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_41_42774_s_401	15302869	1) The inhibitors of PARP-1 and the antisense RNA for PARP-1 mRNA decreased the amounts of AM-PARP and the expression of TNF-alpha and iNOS (Figs.  1,  2,  3) and the LPS-induced DNA binding of NF-kappaB ( Fig. 5).	bind
21581	2	6260	7	NULL	NULL	NULL	NULL	PARP-1mRNA	NucleicAcid	antisense	decrease					AM-PARP	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_41_42774_s_401	15302869	1) The inhibitors of PARP-1 and the antisense RNA for PARP-1 mRNA decreased the amounts of AM-PARP and the expression of TNF-alpha and iNOS (Figs.  1,  2,  3) and the LPS-induced DNA binding of NF-kappaB ( Fig. 5).	bind
21582	3	6260	7	NULL	NULL	NULL	NULL	PARP-1 inhibitor	Chemical		decrease					TNF-alpha	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_41_42774_s_401	15302869	1) The inhibitors of PARP-1 and the antisense RNA for PARP-1 mRNA decreased the amounts of AM-PARP and the expression of TNF-alpha and iNOS (Figs.  1,  2,  3) and the LPS-induced DNA binding of NF-kappaB ( Fig. 5).	bind
21583	4	6260	7	NULL	NULL	NULL	NULL	PARP-1 mRNA	NucleicAcid	antisense	decrease					TNF-alpha	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_41_42774_s_401	15302869	1) The inhibitors of PARP-1 and the antisense RNA for PARP-1 mRNA decreased the amounts of AM-PARP and the expression of TNF-alpha and iNOS (Figs.  1,  2,  3) and the LPS-induced DNA binding of NF-kappaB ( Fig. 5).	bind
21584	5	6260	7	NULL	NULL	NULL	NULL	NF-kappaB	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_41_42774_s_401	15302869	1) The inhibitors of PARP-1 and the antisense RNA for PARP-1 mRNA decreased the amounts of AM-PARP and the expression of TNF-alpha and iNOS (Figs.  1,  2,  3) and the LPS-induced DNA binding of NF-kappaB ( Fig. 5).	bind
21585	6	6260	7	NULL	NULL	NULL	NULL	LPS	Chemical		induce					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_41_42774_s_401	15302869	1) The inhibitors of PARP-1 and the antisense RNA for PARP-1 mRNA decreased the amounts of AM-PARP and the expression of TNF-alpha and iNOS (Figs.  1,  2,  3) and the LPS-induced DNA binding of NF-kappaB ( Fig. 5).	bind
26366	7	6260	7	NULL	NULL	NULL	NULL	PARP-1 inhibitor	Chemical		decrease					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_41_42774_s_401	15302869	1) The inhibitors of PARP-1 and the antisense RNA for PARP-1 mRNA decreased the amounts of AM-PARP and the expression of TNF-alpha and iNOS (Figs.  1,  2,  3) and the LPS-induced DNA binding of NF-kappaB ( Fig. 5).	bind
26367	8	6260	7	NULL	NULL	NULL	NULL	PARP-1 mRNA	NucleicAcid	antisense	decrease					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_41_42774_s_401	15302869	1) The inhibitors of PARP-1 and the antisense RNA for PARP-1 mRNA decreased the amounts of AM-PARP and the expression of TNF-alpha and iNOS (Figs.  1,  2,  3) and the LPS-induced DNA binding of NF-kappaB ( Fig. 5).	bind
26369	10	6260	7	NULL	NULL	NULL	NULL	PARP-1 mRNA	NucleicAcid	antisense	decrease					iNOS	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_41_42774_s_401	15302869	1) The inhibitors of PARP-1 and the antisense RNA for PARP-1 mRNA decreased the amounts of AM-PARP and the expression of TNF-alpha and iNOS (Figs.  1,  2,  3) and the LPS-induced DNA binding of NF-kappaB ( Fig. 5).	bind
26372	11	6260	7	NULL	NULL	NULL	NULL	PARP-1 inhibitor	Chemical		decrease					 iNOS	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_41_42774_s_401	15302869	1) The inhibitors of PARP-1 and the antisense RNA for PARP-1 mRNA decreased the amounts of AM-PARP and the expression of TNF-alpha and iNOS (Figs.  1,  2,  3) and the LPS-induced DNA binding of NF-kappaB ( Fig. 5).	bind
19258	1	6261	5	NULL	NULL	0	NULL	myosin molecules	NULL		udergoes	NULL				post-translational modifications	NULL	differential			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_18_15117_s_282	11134017	1) The myosin molecules are biochemically heterogeneous as a result of differential post-translational modifications; 2) the  Drosophila myosins occupy a wider range of functionally active molecular orientations in the way they are deposited on the third bead substrate, some of which restrict the production of the full displacement; or 3) the myosin step size depends upon the geometry of myosin binding to actin and the degrees of freedom of movement within the myosin molecule.	bind
19259	2	6261	5	NULL	NULL	0	NULL	statement 1	NULL		results in	NULL				biochemically heterogeneous myosin molecules	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_18_15117_s_282	11134017	1) The myosin molecules are biochemically heterogeneous as a result of differential post-translational modifications; 2) the  Drosophila myosins occupy a wider range of functionally active molecular orientations in the way they are deposited on the third bead substrate, some of which restrict the production of the full displacement; or 3) the myosin step size depends upon the geometry of myosin binding to actin and the degrees of freedom of movement within the myosin molecule.	bind
19260	3	6261	5	10	NULL	0	NULL	myosins	NULL	Drosophila	occupy	NULL				molecular orientations	NULL	functionally active			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_15117_s_282	11134017	1) The myosin molecules are biochemically heterogeneous as a result of differential post-translational modifications; 2) the  Drosophila myosins occupy a wider range of functionally active molecular orientations in the way they are deposited on the third bead substrate, some of which restrict the production of the full displacement; or 3) the myosin step size depends upon the geometry of myosin binding to actin and the degrees of freedom of movement within the myosin molecule.	bind
19261	4	6261	5	NULL	NULL	0	NULL	myosin	NULL		bind	NULL				actin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_18_15117_s_282	11134017	1) The myosin molecules are biochemically heterogeneous as a result of differential post-translational modifications; 2) the  Drosophila myosins occupy a wider range of functionally active molecular orientations in the way they are deposited on the third bead substrate, some of which restrict the production of the full displacement; or 3) the myosin step size depends upon the geometry of myosin binding to actin and the degrees of freedom of movement within the myosin molecule.	bind
19262	5	6261	5	NULL	NULL	0	NULL	myosin step size	NULL		depends upon	NULL				statement 4	NULL	geometry of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_18_15117_s_282	11134017	1) The myosin molecules are biochemically heterogeneous as a result of differential post-translational modifications; 2) the  Drosophila myosins occupy a wider range of functionally active molecular orientations in the way they are deposited on the third bead substrate, some of which restrict the production of the full displacement; or 3) the myosin step size depends upon the geometry of myosin binding to actin and the degrees of freedom of movement within the myosin molecule.	bind
21586	1	6261	7	NULL	NULL	NULL	NULL	myosin molecules	GP		are					heterogeneous		biochemically			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_15117_s_282	11134017	1) The myosin molecules are biochemically heterogeneous as a result of differential post-translational modifications; 2) the  Drosophila myosins occupy a wider range of functionally active molecular orientations in the way they are deposited on the third bead substrate, some of which restrict the production of the full displacement; or 3) the myosin step size depends upon the geometry of myosin binding to actin and the degrees of freedom of movement within the myosin molecule.	bind
21587	2	6261	7	NULL	NULL	NULL	NULL	statement 1	Process		is because of 					post-translational modifications	Process	differential 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_15117_s_282	11134017	1) The myosin molecules are biochemically heterogeneous as a result of differential post-translational modifications; 2) the  Drosophila myosins occupy a wider range of functionally active molecular orientations in the way they are deposited on the third bead substrate, some of which restrict the production of the full displacement; or 3) the myosin step size depends upon the geometry of myosin binding to actin and the degrees of freedom of movement within the myosin molecule.	bind
21588	3	6261	7	NULL	NULL	NULL	NULL	myosins	GP	Drosophila	are deposited on					third bead substrate	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_15117_s_282	11134017	1) The myosin molecules are biochemically heterogeneous as a result of differential post-translational modifications; 2) the  Drosophila myosins occupy a wider range of functionally active molecular orientations in the way they are deposited on the third bead substrate, some of which restrict the production of the full displacement; or 3) the myosin step size depends upon the geometry of myosin binding to actin and the degrees of freedom of movement within the myosin molecule.	bind
21589	4	6261	7	NULL	NULL	NULL	NULL	myosins	GP	Drosophila	occupy					molecular orientations	Process	functionally active			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_15117_s_282	11134017	1) The myosin molecules are biochemically heterogeneous as a result of differential post-translational modifications; 2) the  Drosophila myosins occupy a wider range of functionally active molecular orientations in the way they are deposited on the third bead substrate, some of which restrict the production of the full displacement; or 3) the myosin step size depends upon the geometry of myosin binding to actin and the degrees of freedom of movement within the myosin molecule.	bind
21590	5	6261	7	NULL	NULL	NULL	NULL	myosin	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_15117_s_282	11134017	1) The myosin molecules are biochemically heterogeneous as a result of differential post-translational modifications; 2) the  Drosophila myosins occupy a wider range of functionally active molecular orientations in the way they are deposited on the third bead substrate, some of which restrict the production of the full displacement; or 3) the myosin step size depends upon the geometry of myosin binding to actin and the degrees of freedom of movement within the myosin molecule.	bind
16895	1	6262	5	NULL	NULL	0	NULL	prothrombin	NULL		bind	NULL				FXI	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_41_31954_s_224	10924522	1) The rA1 domain inhibits the binding of prothrombin to FXI with an IC50 of 4 x 10 7M (Fig.  1 A, Table  I).	bind
16896	2	6262	5	NULL	NULL	0	NULL		NULL		inhibit	NULL		rA1 domain		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_41_31954_s_224	10924522	1) The rA1 domain inhibits the binding of prothrombin to FXI with an IC50 of 4 x 10 7M (Fig.  1 A, Table  I).	bind
21596	1	6262	7	NULL	NULL	NULL	NULL	prothrombin 	GP		bind					FXI	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_31954_s_224	10924522	1) The rA1 domain inhibits the binding of prothrombin to FXI with an IC50 of 4 x 10 7M (Fig.  1 A, Table  I).	bind
21597	2	6262	7	NULL	NULL	NULL	NULL				inhibits			rA1 domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_31954_s_224	10924522	1) The rA1 domain inhibits the binding of prothrombin to FXI with an IC50 of 4 x 10 7M (Fig.  1 A, Table  I).	bind
19222	1	6263	5	NULL	NULL	0	NULL	FKHRL1	NULL		contains	NULL			regulatory region of promoter		NULL			insulin-responsive sequence-like sequences	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39152_s_260	10995739	1) The regulatory region of the promoter of the Fas ligand gene contains three insulin-responsive sequence-like sequences for FKHRL1, and the binding of FKHRL1 to these sequences enhances the transcription of the Fas ligand ( 51); 2) the removal of growth factors from culture medium up-regulates the expression of Fas ligand mRNA and protein and stimulates apoptosis in several cell lines, including PC12 cells and primary cultured neurons ( 52); and 3) the stimulation of PC12 cells with a survival factor as shown in the present study activates PI3K/Akt kinase and increases the phosphorylation of FKHRL1, which was shown to inhibit the expression of the Fas ligand in fibroblasts ( 21,  52).	bind
19223	2	6263	5	NULL	NULL	0	NULL	FKHRL1	NULL		bind	NULL				Fas ligand gene	NULL			insulin-responsive sequence-like sequences	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_50_39152_s_260	10995739	1) The regulatory region of the promoter of the Fas ligand gene contains three insulin-responsive sequence-like sequences for FKHRL1, and the binding of FKHRL1 to these sequences enhances the transcription of the Fas ligand ( 51); 2) the removal of growth factors from culture medium up-regulates the expression of Fas ligand mRNA and protein and stimulates apoptosis in several cell lines, including PC12 cells and primary cultured neurons ( 52); and 3) the stimulation of PC12 cells with a survival factor as shown in the present study activates PI3K/Akt kinase and increases the phosphorylation of FKHRL1, which was shown to inhibit the expression of the Fas ligand in fibroblasts ( 21,  52).	bind
19224	3	6263	5	NULL	NULL	0	NULL	statement 2	NULL		enhances	NULL				Fas ligand	NULL	transcription of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_50_39152_s_260	10995739	1) The regulatory region of the promoter of the Fas ligand gene contains three insulin-responsive sequence-like sequences for FKHRL1, and the binding of FKHRL1 to these sequences enhances the transcription of the Fas ligand ( 51); 2) the removal of growth factors from culture medium up-regulates the expression of Fas ligand mRNA and protein and stimulates apoptosis in several cell lines, including PC12 cells and primary cultured neurons ( 52); and 3) the stimulation of PC12 cells with a survival factor as shown in the present study activates PI3K/Akt kinase and increases the phosphorylation of FKHRL1, which was shown to inhibit the expression of the Fas ligand in fibroblasts ( 21,  52).	bind
19225	4	6263	5	NULL	NULL	0	NULL	growth factors	NULL	removal of	up-regulates	NULL				Fas ligand mRNA	NULL	expression of			NULL	culture medium	0	NULL	NULL	NULL	gw60_jbiolchem_275_50_39152_s_260	10995739	1) The regulatory region of the promoter of the Fas ligand gene contains three insulin-responsive sequence-like sequences for FKHRL1, and the binding of FKHRL1 to these sequences enhances the transcription of the Fas ligand ( 51); 2) the removal of growth factors from culture medium up-regulates the expression of Fas ligand mRNA and protein and stimulates apoptosis in several cell lines, including PC12 cells and primary cultured neurons ( 52); and 3) the stimulation of PC12 cells with a survival factor as shown in the present study activates PI3K/Akt kinase and increases the phosphorylation of FKHRL1, which was shown to inhibit the expression of the Fas ligand in fibroblasts ( 21,  52).	bind
19226	5	6263	5	NULL	NULL	0	NULL	growth factors	NULL	removal of	up-regulates	NULL				Fas ligand protein	NULL	expression of			NULL	culture medium	0	NULL	NULL	NULL	gw60_jbiolchem_275_50_39152_s_260	10995739	1) The regulatory region of the promoter of the Fas ligand gene contains three insulin-responsive sequence-like sequences for FKHRL1, and the binding of FKHRL1 to these sequences enhances the transcription of the Fas ligand ( 51); 2) the removal of growth factors from culture medium up-regulates the expression of Fas ligand mRNA and protein and stimulates apoptosis in several cell lines, including PC12 cells and primary cultured neurons ( 52); and 3) the stimulation of PC12 cells with a survival factor as shown in the present study activates PI3K/Akt kinase and increases the phosphorylation of FKHRL1, which was shown to inhibit the expression of the Fas ligand in fibroblasts ( 21,  52).	bind
19227	6	6263	5	NULL	NULL	0	NULL	statement 4	NULL		stimulates	NULL				apoptosis	NULL				NULL	PC12 cells	0	NULL	NULL	NULL	gw60_jbiolchem_275_50_39152_s_260	10995739	1) The regulatory region of the promoter of the Fas ligand gene contains three insulin-responsive sequence-like sequences for FKHRL1, and the binding of FKHRL1 to these sequences enhances the transcription of the Fas ligand ( 51); 2) the removal of growth factors from culture medium up-regulates the expression of Fas ligand mRNA and protein and stimulates apoptosis in several cell lines, including PC12 cells and primary cultured neurons ( 52); and 3) the stimulation of PC12 cells with a survival factor as shown in the present study activates PI3K/Akt kinase and increases the phosphorylation of FKHRL1, which was shown to inhibit the expression of the Fas ligand in fibroblasts ( 21,  52).	bind
19228	7	6263	5	NULL	NULL	0	NULL	statement 4	NULL		stimulates	NULL				apoptosis	NULL				NULL	primary cultured neurons	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39152_s_260	10995739	1) The regulatory region of the promoter of the Fas ligand gene contains three insulin-responsive sequence-like sequences for FKHRL1, and the binding of FKHRL1 to these sequences enhances the transcription of the Fas ligand ( 51); 2) the removal of growth factors from culture medium up-regulates the expression of Fas ligand mRNA and protein and stimulates apoptosis in several cell lines, including PC12 cells and primary cultured neurons ( 52); and 3) the stimulation of PC12 cells with a survival factor as shown in the present study activates PI3K/Akt kinase and increases the phosphorylation of FKHRL1, which was shown to inhibit the expression of the Fas ligand in fibroblasts ( 21,  52).	bind
19229	8	6263	5	NULL	NULL	0	NULL	statement 5	NULL		stimulates	NULL				apoptosis	NULL				NULL	PC12 cells	0	NULL	NULL	NULL	gw60_jbiolchem_275_50_39152_s_260	10995739	1) The regulatory region of the promoter of the Fas ligand gene contains three insulin-responsive sequence-like sequences for FKHRL1, and the binding of FKHRL1 to these sequences enhances the transcription of the Fas ligand ( 51); 2) the removal of growth factors from culture medium up-regulates the expression of Fas ligand mRNA and protein and stimulates apoptosis in several cell lines, including PC12 cells and primary cultured neurons ( 52); and 3) the stimulation of PC12 cells with a survival factor as shown in the present study activates PI3K/Akt kinase and increases the phosphorylation of FKHRL1, which was shown to inhibit the expression of the Fas ligand in fibroblasts ( 21,  52).	bind
19230	9	6263	5	NULL	NULL	0	NULL	statement 5	NULL		stimulates	NULL				apoptosis	NULL				NULL	primary cultured neurons	0	NULL	NULL	NULL	gw60_jbiolchem_275_50_39152_s_260	10995739	1) The regulatory region of the promoter of the Fas ligand gene contains three insulin-responsive sequence-like sequences for FKHRL1, and the binding of FKHRL1 to these sequences enhances the transcription of the Fas ligand ( 51); 2) the removal of growth factors from culture medium up-regulates the expression of Fas ligand mRNA and protein and stimulates apoptosis in several cell lines, including PC12 cells and primary cultured neurons ( 52); and 3) the stimulation of PC12 cells with a survival factor as shown in the present study activates PI3K/Akt kinase and increases the phosphorylation of FKHRL1, which was shown to inhibit the expression of the Fas ligand in fibroblasts ( 21,  52).	bind
19231	10	6263	5	NULL	NULL	0	NULL	survival factor	NULL		stimulates	NULL				PC12 cells	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_50_39152_s_260	10995739	1) The regulatory region of the promoter of the Fas ligand gene contains three insulin-responsive sequence-like sequences for FKHRL1, and the binding of FKHRL1 to these sequences enhances the transcription of the Fas ligand ( 51); 2) the removal of growth factors from culture medium up-regulates the expression of Fas ligand mRNA and protein and stimulates apoptosis in several cell lines, including PC12 cells and primary cultured neurons ( 52); and 3) the stimulation of PC12 cells with a survival factor as shown in the present study activates PI3K/Akt kinase and increases the phosphorylation of FKHRL1, which was shown to inhibit the expression of the Fas ligand in fibroblasts ( 21,  52).	bind
19232	11	6263	5	NULL	NULL	0	NULL	statement 10	NULL		activates	NULL				PI3K/Akt kinase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_50_39152_s_260	10995739	1) The regulatory region of the promoter of the Fas ligand gene contains three insulin-responsive sequence-like sequences for FKHRL1, and the binding of FKHRL1 to these sequences enhances the transcription of the Fas ligand ( 51); 2) the removal of growth factors from culture medium up-regulates the expression of Fas ligand mRNA and protein and stimulates apoptosis in several cell lines, including PC12 cells and primary cultured neurons ( 52); and 3) the stimulation of PC12 cells with a survival factor as shown in the present study activates PI3K/Akt kinase and increases the phosphorylation of FKHRL1, which was shown to inhibit the expression of the Fas ligand in fibroblasts ( 21,  52).	bind
19233	12	6263	5	NULL	NULL	0	NULL	statement 10	NULL		increases	NULL				FKHRL1	NULL	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_50_39152_s_260	10995739	1) The regulatory region of the promoter of the Fas ligand gene contains three insulin-responsive sequence-like sequences for FKHRL1, and the binding of FKHRL1 to these sequences enhances the transcription of the Fas ligand ( 51); 2) the removal of growth factors from culture medium up-regulates the expression of Fas ligand mRNA and protein and stimulates apoptosis in several cell lines, including PC12 cells and primary cultured neurons ( 52); and 3) the stimulation of PC12 cells with a survival factor as shown in the present study activates PI3K/Akt kinase and increases the phosphorylation of FKHRL1, which was shown to inhibit the expression of the Fas ligand in fibroblasts ( 21,  52).	bind
19234	13	6263	5	NULL	NULL	0	NULL	statement 12	NULL		inhibit	NULL				Fas ligand	NULL	expression of			NULL	fibroblasts	0	NULL	NULL	NULL	gw60_jbiolchem_275_50_39152_s_260	10995739	1) The regulatory region of the promoter of the Fas ligand gene contains three insulin-responsive sequence-like sequences for FKHRL1, and the binding of FKHRL1 to these sequences enhances the transcription of the Fas ligand ( 51); 2) the removal of growth factors from culture medium up-regulates the expression of Fas ligand mRNA and protein and stimulates apoptosis in several cell lines, including PC12 cells and primary cultured neurons ( 52); and 3) the stimulation of PC12 cells with a survival factor as shown in the present study activates PI3K/Akt kinase and increases the phosphorylation of FKHRL1, which was shown to inhibit the expression of the Fas ligand in fibroblasts ( 21,  52).	bind
21600	1	6263	7	NULL	NULL	NULL	NULL	Fas ligand gene	GP		contains				regulatory region of promoter	FKHRL1	GP			 insulin-responsive sequences	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39152_s_260	10995739	1) The regulatory region of the promoter of the Fas ligand gene contains three insulin-responsive sequence-like sequences for FKHRL1, and the binding of FKHRL1 to these sequences enhances the transcription of the Fas ligand ( 51); 2) the removal of growth factors from culture medium up-regulates the expression of Fas ligand mRNA and protein and stimulates apoptosis in several cell lines, including PC12 cells and primary cultured neurons ( 52); and 3) the stimulation of PC12 cells with a survival factor as shown in the present study activates PI3K/Akt kinase and increases the phosphorylation of FKHRL1, which was shown to inhibit the expression of the Fas ligand in fibroblasts ( 21,  52).	bind
21602	2	6263	7	NULL	NULL	NULL	NULL				bind			FKHRL1 sequence	 	Fas ligand gene	GP			insulin-responsive sequence	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39152_s_260	10995739	1) The regulatory region of the promoter of the Fas ligand gene contains three insulin-responsive sequence-like sequences for FKHRL1, and the binding of FKHRL1 to these sequences enhances the transcription of the Fas ligand ( 51); 2) the removal of growth factors from culture medium up-regulates the expression of Fas ligand mRNA and protein and stimulates apoptosis in several cell lines, including PC12 cells and primary cultured neurons ( 52); and 3) the stimulation of PC12 cells with a survival factor as shown in the present study activates PI3K/Akt kinase and increases the phosphorylation of FKHRL1, which was shown to inhibit the expression of the Fas ligand in fibroblasts ( 21,  52).	bind
21604	3	6263	7	NULL	NULL	NULL	NULL	statement 2	Process		enhance					Fas ligand	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39152_s_260	10995739	1) The regulatory region of the promoter of the Fas ligand gene contains three insulin-responsive sequence-like sequences for FKHRL1, and the binding of FKHRL1 to these sequences enhances the transcription of the Fas ligand ( 51); 2) the removal of growth factors from culture medium up-regulates the expression of Fas ligand mRNA and protein and stimulates apoptosis in several cell lines, including PC12 cells and primary cultured neurons ( 52); and 3) the stimulation of PC12 cells with a survival factor as shown in the present study activates PI3K/Akt kinase and increases the phosphorylation of FKHRL1, which was shown to inhibit the expression of the Fas ligand in fibroblasts ( 21,  52).	bind
21605	4	6263	7	NULL	NULL	NULL	NULL	growth factors	GP	removal of 	upregulates					Fas ligand mRNA 	NucleicAcid	the expression of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39152_s_260	10995739	1) The regulatory region of the promoter of the Fas ligand gene contains three insulin-responsive sequence-like sequences for FKHRL1, and the binding of FKHRL1 to these sequences enhances the transcription of the Fas ligand ( 51); 2) the removal of growth factors from culture medium up-regulates the expression of Fas ligand mRNA and protein and stimulates apoptosis in several cell lines, including PC12 cells and primary cultured neurons ( 52); and 3) the stimulation of PC12 cells with a survival factor as shown in the present study activates PI3K/Akt kinase and increases the phosphorylation of FKHRL1, which was shown to inhibit the expression of the Fas ligand in fibroblasts ( 21,  52).	bind
21606	5	6263	7	NULL	NULL	NULL	NULL	growth factors	GP	removal of	upregulates					Fas ligand protein	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39152_s_260	10995739	1) The regulatory region of the promoter of the Fas ligand gene contains three insulin-responsive sequence-like sequences for FKHRL1, and the binding of FKHRL1 to these sequences enhances the transcription of the Fas ligand ( 51); 2) the removal of growth factors from culture medium up-regulates the expression of Fas ligand mRNA and protein and stimulates apoptosis in several cell lines, including PC12 cells and primary cultured neurons ( 52); and 3) the stimulation of PC12 cells with a survival factor as shown in the present study activates PI3K/Akt kinase and increases the phosphorylation of FKHRL1, which was shown to inhibit the expression of the Fas ligand in fibroblasts ( 21,  52).	bind
21607	6	6263	7	NULL	NULL	NULL	NULL	statement 4	Process		stimulate					apoptosis	Process				NULL	in PC12 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39152_s_260	10995739	1) The regulatory region of the promoter of the Fas ligand gene contains three insulin-responsive sequence-like sequences for FKHRL1, and the binding of FKHRL1 to these sequences enhances the transcription of the Fas ligand ( 51); 2) the removal of growth factors from culture medium up-regulates the expression of Fas ligand mRNA and protein and stimulates apoptosis in several cell lines, including PC12 cells and primary cultured neurons ( 52); and 3) the stimulation of PC12 cells with a survival factor as shown in the present study activates PI3K/Akt kinase and increases the phosphorylation of FKHRL1, which was shown to inhibit the expression of the Fas ligand in fibroblasts ( 21,  52).	bind
21608	7	6263	7	NULL	NULL	NULL	NULL	statement 5	Process		stimulate					apoptosis	Process				NULL	primary cultured neurons 	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39152_s_260	10995739	1) The regulatory region of the promoter of the Fas ligand gene contains three insulin-responsive sequence-like sequences for FKHRL1, and the binding of FKHRL1 to these sequences enhances the transcription of the Fas ligand ( 51); 2) the removal of growth factors from culture medium up-regulates the expression of Fas ligand mRNA and protein and stimulates apoptosis in several cell lines, including PC12 cells and primary cultured neurons ( 52); and 3) the stimulation of PC12 cells with a survival factor as shown in the present study activates PI3K/Akt kinase and increases the phosphorylation of FKHRL1, which was shown to inhibit the expression of the Fas ligand in fibroblasts ( 21,  52).	bind
21609	8	6263	7	NULL	NULL	NULL	NULL	statement 4	Process		stimulate					apoptosis	Process				NULL	primary cultured neurons 	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39152_s_260	10995739	1) The regulatory region of the promoter of the Fas ligand gene contains three insulin-responsive sequence-like sequences for FKHRL1, and the binding of FKHRL1 to these sequences enhances the transcription of the Fas ligand ( 51); 2) the removal of growth factors from culture medium up-regulates the expression of Fas ligand mRNA and protein and stimulates apoptosis in several cell lines, including PC12 cells and primary cultured neurons ( 52); and 3) the stimulation of PC12 cells with a survival factor as shown in the present study activates PI3K/Akt kinase and increases the phosphorylation of FKHRL1, which was shown to inhibit the expression of the Fas ligand in fibroblasts ( 21,  52).	bind
21610	9	6263	7	NULL	NULL	NULL	NULL	statement 5	Process		stimulate					apoptosis	Process				NULL	in PC12 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39152_s_260	10995739	1) The regulatory region of the promoter of the Fas ligand gene contains three insulin-responsive sequence-like sequences for FKHRL1, and the binding of FKHRL1 to these sequences enhances the transcription of the Fas ligand ( 51); 2) the removal of growth factors from culture medium up-regulates the expression of Fas ligand mRNA and protein and stimulates apoptosis in several cell lines, including PC12 cells and primary cultured neurons ( 52); and 3) the stimulation of PC12 cells with a survival factor as shown in the present study activates PI3K/Akt kinase and increases the phosphorylation of FKHRL1, which was shown to inhibit the expression of the Fas ligand in fibroblasts ( 21,  52).	bind
21611	10	6263	7	NULL	NULL	NULL	NULL	PC12 cells with survival factor 	Cell	stimulation of	activates					PI3K/Akt kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39152_s_260	10995739	1) The regulatory region of the promoter of the Fas ligand gene contains three insulin-responsive sequence-like sequences for FKHRL1, and the binding of FKHRL1 to these sequences enhances the transcription of the Fas ligand ( 51); 2) the removal of growth factors from culture medium up-regulates the expression of Fas ligand mRNA and protein and stimulates apoptosis in several cell lines, including PC12 cells and primary cultured neurons ( 52); and 3) the stimulation of PC12 cells with a survival factor as shown in the present study activates PI3K/Akt kinase and increases the phosphorylation of FKHRL1, which was shown to inhibit the expression of the Fas ligand in fibroblasts ( 21,  52).	bind
21612	11	6263	7	NULL	NULL	NULL	NULL	statement 10	Process		increases					FKHRL1	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39152_s_260	10995739	1) The regulatory region of the promoter of the Fas ligand gene contains three insulin-responsive sequence-like sequences for FKHRL1, and the binding of FKHRL1 to these sequences enhances the transcription of the Fas ligand ( 51); 2) the removal of growth factors from culture medium up-regulates the expression of Fas ligand mRNA and protein and stimulates apoptosis in several cell lines, including PC12 cells and primary cultured neurons ( 52); and 3) the stimulation of PC12 cells with a survival factor as shown in the present study activates PI3K/Akt kinase and increases the phosphorylation of FKHRL1, which was shown to inhibit the expression of the Fas ligand in fibroblasts ( 21,  52).	bind
21613	12	6263	7	NULL	NULL	NULL	NULL	statement 11	Process		inhibits					Fas ligand	GP	the expression of			NULL	in fibroblasts	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39152_s_260	10995739	1) The regulatory region of the promoter of the Fas ligand gene contains three insulin-responsive sequence-like sequences for FKHRL1, and the binding of FKHRL1 to these sequences enhances the transcription of the Fas ligand ( 51); 2) the removal of growth factors from culture medium up-regulates the expression of Fas ligand mRNA and protein and stimulates apoptosis in several cell lines, including PC12 cells and primary cultured neurons ( 52); and 3) the stimulation of PC12 cells with a survival factor as shown in the present study activates PI3K/Akt kinase and increases the phosphorylation of FKHRL1, which was shown to inhibit the expression of the Fas ligand in fibroblasts ( 21,  52).	bind
19216	1	6264	5	NULL	NULL	0	NULL	Sp1	NULL		bind	NULL				PII	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_25_14692_s_103	8663083	1) The size of the nuclear factor that enhances Sp1 binding to PII is about 38-42 kDa, the size of the catalytic subunit of PP1; and 2) glucose-mediated activation of Sp1 binding to PII is OA-sensitive at a concentration suggesting the factor to be a PP1-like activity.	bind
19217	2	6264	5	NULL	NULL	0	NULL	nuclear factor	NULL		enhances	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_25_14692_s_103	8663083	1) The size of the nuclear factor that enhances Sp1 binding to PII is about 38-42 kDa, the size of the catalytic subunit of PP1; and 2) glucose-mediated activation of Sp1 binding to PII is OA-sensitive at a concentration suggesting the factor to be a PP1-like activity.	bind
19218	3	6264	5	NULL	NULL	0	NULL	glucose	NULL		mediate	NULL				statement 1	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_25_14692_s_103	8663083	1) The size of the nuclear factor that enhances Sp1 binding to PII is about 38-42 kDa, the size of the catalytic subunit of PP1; and 2) glucose-mediated activation of Sp1 binding to PII is OA-sensitive at a concentration suggesting the factor to be a PP1-like activity.	bind
19219	4	6264	5	NULL	NULL	0	NULL	statement 3	NULL		is sensitive to	NULL				OA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_25_14692_s_103	8663083	1) The size of the nuclear factor that enhances Sp1 binding to PII is about 38-42 kDa, the size of the catalytic subunit of PP1; and 2) glucose-mediated activation of Sp1 binding to PII is OA-sensitive at a concentration suggesting the factor to be a PP1-like activity.	bind
19220	5	6264	5	NULL	NULL	0	NULL	nuclear factor	NULL		has	NULL				PP1-like activity	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_25_14692_s_103	8663083	1) The size of the nuclear factor that enhances Sp1 binding to PII is about 38-42 kDa, the size of the catalytic subunit of PP1; and 2) glucose-mediated activation of Sp1 binding to PII is OA-sensitive at a concentration suggesting the factor to be a PP1-like activity.	bind
19221	6	6264	5	NULL	NULL	0	NULL	statement 4	NULL		suggests	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_25_14692_s_103	8663083	1) The size of the nuclear factor that enhances Sp1 binding to PII is about 38-42 kDa, the size of the catalytic subunit of PP1; and 2) glucose-mediated activation of Sp1 binding to PII is OA-sensitive at a concentration suggesting the factor to be a PP1-like activity.	bind
21614	1	6264	7	NULL	NULL	NULL	NULL	Sp1	GP		bind					PII	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_25_14692_s_103	8663083	1) The size of the nuclear factor that enhances Sp1 binding to PII is about 38-42 kDa, the size of the catalytic subunit of PP1; and 2) glucose-mediated activation of Sp1 binding to PII is OA-sensitive at a concentration suggesting the factor to be a PP1-like activity.	bind
21615	2	6264	7	NULL	NULL	NULL	NULL	nuclear factor	GP		enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_25_14692_s_103	8663083	1) The size of the nuclear factor that enhances Sp1 binding to PII is about 38-42 kDa, the size of the catalytic subunit of PP1; and 2) glucose-mediated activation of Sp1 binding to PII is OA-sensitive at a concentration suggesting the factor to be a PP1-like activity.	bind
21616	3	6264	7	NULL	NULL	NULL	NULL	glucose	Chemical		mediates					statement 1	Process	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_25_14692_s_103	8663083	1) The size of the nuclear factor that enhances Sp1 binding to PII is about 38-42 kDa, the size of the catalytic subunit of PP1; and 2) glucose-mediated activation of Sp1 binding to PII is OA-sensitive at a concentration suggesting the factor to be a PP1-like activity.	bind
21617	4	6264	7	NULL	NULL	NULL	NULL	statement 3	Process		is sensitive to					OA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_25_14692_s_103	8663083	1) The size of the nuclear factor that enhances Sp1 binding to PII is about 38-42 kDa, the size of the catalytic subunit of PP1; and 2) glucose-mediated activation of Sp1 binding to PII is OA-sensitive at a concentration suggesting the factor to be a PP1-like activity.	bind
19215	1	6265	5	NULL	NULL	0	NULL	ouabain	NULL		bind	NULL				phosphoenzyme	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_45_31792_s_110	10542201	1) The stoichiometries of ATP binding ( 15,  24), rubidium occlusion (Fig.  2) and phosphorylation by ATP ( 10), Pi ( 14), acetyl phosphate ( 16), and  p-nitrophenyl phosphate ( 14) and the ratio of ouabain binding to phosphoenzyme ( 15,  24); 2) half-site reactivities of Na E1P to acetate ( 16) and  p-nitrophenol ( 15), namely a quarter site reactivity of the alpha-chain ( 10); 3) the fact that ATP induced four different conformational changes out of phase ( 11); 4) 32P binding and the burst size of Pi (Fig.  3,  B and  C); and 5) electron microscopy (Fig.  4).	bind
21622	1	6265	7	NULL	NULL	NULL	NULL	ouabain	GP		bind					phosphoenzyme	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_45_31792_s_110	10542201	1) The stoichiometries of ATP binding ( 15,  24), rubidium occlusion (Fig.  2) and phosphorylation by ATP ( 10), Pi ( 14), acetyl phosphate ( 16), and  p-nitrophenyl phosphate ( 14) and the ratio of ouabain binding to phosphoenzyme ( 15,  24); 2) half-site reactivities of Na E1P to acetate ( 16) and  p-nitrophenol ( 15), namely a quarter site reactivity of the alpha-chain ( 10); 3) the fact that ATP induced four different conformational changes out of phase ( 11); 4) 32P binding and the burst size of Pi (Fig.  3,  B and  C); and 5) electron microscopy (Fig.  4).	bind
16897	1	6266	5	NULL	NULL	0	NULL	TSG101	NULL		bind	NULL		N-terminal UEV domain			NULL		P(S/T)AP peptide motifs		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_34_36059_s_31	15218037	1) The TSG101 N-terminal UEV domain binds P(S/T)AP peptide motifs.	bind
21629	1	6266	7	NULL	NULL	NULL	NULL	TSG101	GP		binds			N-terminal UEV domain					P(S/T)AP peptide motifs		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_34_36059_s_31	15218037	1) The TSG101 N-terminal UEV domain binds P(S/T)AP peptide motifs.	bind
16898	1	6267	5	10	NULL	0	NULL	Transducin	NULL		bind	NULL				RGS9d	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_40_37365_s_245	11495924	1) Transducin binds demonstrably to RGS9d, but the difference between the binding with and without PDEgamma is small.	bind
21634	1	6267	7	NULL	NULL	NULL	NULL	Transducin	GP		binds					RGS9d	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_40_37365_s_245	11495924	1) Transducin binds demonstrably to RGS9d, but the difference between the binding with and without PDEgamma is small.	bind
16899	1	6268	5	10	NULL	0	NULL	tropomyosin molecules			bind					actin					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_43_25455_s_179	7592713	1) Troponin  greatly promotes the binding of individual tropomyosin molecules to  actin, regardless of the Ca   concentration.	bind
16900	2	6268	5	NULL	NULL	0	NULL	Troponin	NULL		promotes	NULL	greatly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_43_25455_s_179	7592713	1) Troponin  greatly promotes the binding of individual tropomyosin molecules to  actin, regardless of the Ca   concentration.	bind
16901	3	6268	5	NULL	NULL	0	NULL	statement 2	NULL		is independent of	NULL				Ca 	NULL	concentration of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_43_25455_s_179	7592713	1) Troponin  greatly promotes the binding of individual tropomyosin molecules to  actin, regardless of the Ca   concentration.	bind
21638	1	6268	7	NULL	NULL	NULL	NULL	tropomyosin molecules	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_43_25455_s_179	7592713	1) Troponin  greatly promotes the binding of individual tropomyosin molecules to  actin, regardless of the Ca   concentration.	bind
21639	2	6268	7	NULL	NULL	NULL	NULL	Troponin	GP		promotes		greatly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_43_25455_s_179	7592713	1) Troponin  greatly promotes the binding of individual tropomyosin molecules to  actin, regardless of the Ca   concentration.	bind
21640	3	6268	7	NULL	NULL	NULL	NULL	statement 2	Process		is independent of					Ca	Chemical	 concentration 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_43_25455_s_179	7592713	1) Troponin  greatly promotes the binding of individual tropomyosin molecules to  actin, regardless of the Ca   concentration.	bind
16902	1	6269	5	NULL	NULL	0	NULL	uPA	NULL		bind	NULL				uPAR	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_32_29863_s_292	12754207	1) uPA binds to uPAR,  2) uPAR then binds to alpha5beta1 in cis, and 3)  signal transduction is mediated through alpha5beta1  ( Fig. 8).	bind
16903	2	6269	5	NULL	NULL	0	NULL	uPAR	NULL		bind	NULL				alpha5beta1	NULL	in cis			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_32_29863_s_292	12754207	1) uPA binds to uPAR,  2) uPAR then binds to alpha5beta1 in cis, and 3)  signal transduction is mediated through alpha5beta1  ( Fig. 8).	bind
16904	3	6269	5	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_32_29863_s_292	12754207	1) uPA binds to uPAR,  2) uPAR then binds to alpha5beta1 in cis, and 3)  signal transduction is mediated through alpha5beta1  ( Fig. 8).	bind
16905	4	6269	5	NULL	NULL	0	NULL	alpha5beta1	NULL		mediate	NULL				signal transduction	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_32_29863_s_292	12754207	1) uPA binds to uPAR,  2) uPAR then binds to alpha5beta1 in cis, and 3)  signal transduction is mediated through alpha5beta1  ( Fig. 8).	bind
21641	1	6269	7	NULL	NULL	NULL	NULL	uPA	GP		binds to					uPAR	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_32_29863_s_292	12754207	1) uPA binds to uPAR,  2) uPAR then binds to alpha5beta1 in cis, and 3)  signal transduction is mediated through alpha5beta1  ( Fig. 8).	bind
21642	2	6269	7	NULL	NULL	NULL	NULL	uPAR	GP		binds to					alpha5beta1	GP	cis			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_32_29863_s_292	12754207	1) uPA binds to uPAR,  2) uPAR then binds to alpha5beta1 in cis, and 3)  signal transduction is mediated through alpha5beta1  ( Fig. 8).	bind
21643	3	6269	7	NULL	NULL	NULL	NULL	signal transduction	Process		is mediated through					alpha5beta1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_32_29863_s_292	12754207	1) uPA binds to uPAR,  2) uPAR then binds to alpha5beta1 in cis, and 3)  signal transduction is mediated through alpha5beta1  ( Fig. 8).	bind
26375	4	6269	7	NULL	NULL	NULL	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_32_29863_s_292	12754207	1) uPA binds to uPAR,  2) uPAR then binds to alpha5beta1 in cis, and 3)  signal transduction is mediated through alpha5beta1  ( Fig. 8).	bind
16906	1	6270	5	NULL	NULL	0	NULL	Vx	NULL		bind	NULL					NULL		N1 site		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_31_21924_s_233	16754673	1) Vx bound to the N1 and V1 site is rapidly (within 10-20 min) convertible to Zx. 2) Vx bound to the L2 site is either slowly (within hours) or not convertible to Zx. 3) Vx bound to L1 (only in recombinant proteins) is not convertible to Zx.	bind
16907	2	6270	5	NULL	NULL	0	NULL	Vx	NULL		bind	NULL					NULL		V1 site		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_31_21924_s_233	16754673	1) Vx bound to the N1 and V1 site is rapidly (within 10-20 min) convertible to Zx. 2) Vx bound to the L2 site is either slowly (within hours) or not convertible to Zx. 3) Vx bound to L1 (only in recombinant proteins) is not convertible to Zx.	bind
16908	3	6270	5	NULL	NULL	0	NULL	statement 1	NULL		is convertible to	NULL	rapidly			Zx	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_31_21924_s_233	16754673	1) Vx bound to the N1 and V1 site is rapidly (within 10-20 min) convertible to Zx. 2) Vx bound to the L2 site is either slowly (within hours) or not convertible to Zx. 3) Vx bound to L1 (only in recombinant proteins) is not convertible to Zx.	bind
16909	4	6270	5	NULL	NULL	0	NULL	statement 2	NULL		is convertible to	NULL	rapidly			Zx	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_31_21924_s_233	16754673	1) Vx bound to the N1 and V1 site is rapidly (within 10-20 min) convertible to Zx. 2) Vx bound to the L2 site is either slowly (within hours) or not convertible to Zx. 3) Vx bound to L1 (only in recombinant proteins) is not convertible to Zx.	bind
16910	5	6270	5	NULL	NULL	0	NULL	Vx	NULL		bind	NULL					NULL		L2 site		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_31_21924_s_233	16754673	1) Vx bound to the N1 and V1 site is rapidly (within 10-20 min) convertible to Zx. 2) Vx bound to the L2 site is either slowly (within hours) or not convertible to Zx. 3) Vx bound to L1 (only in recombinant proteins) is not convertible to Zx.	bind
16911	6	6270	5	NULL	NULL	0	NULL	statement 5	NULL		is convertible to	NULL	slowly			Zx	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_31_21924_s_233	16754673	1) Vx bound to the N1 and V1 site is rapidly (within 10-20 min) convertible to Zx. 2) Vx bound to the L2 site is either slowly (within hours) or not convertible to Zx. 3) Vx bound to L1 (only in recombinant proteins) is not convertible to Zx.	bind
16912	7	6270	5	NULL	NULL	0	NULL	statement 5	NULL		is not convertible to	NULL				Zx	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_31_21924_s_233	16754673	1) Vx bound to the N1 and V1 site is rapidly (within 10-20 min) convertible to Zx. 2) Vx bound to the L2 site is either slowly (within hours) or not convertible to Zx. 3) Vx bound to L1 (only in recombinant proteins) is not convertible to Zx.	bind
16913	8	6270	5	NULL	NULL	0	NULL	Vx	NULL		bind	NULL	only				NULL	recombinant	L1		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_31_21924_s_233	16754673	1) Vx bound to the N1 and V1 site is rapidly (within 10-20 min) convertible to Zx. 2) Vx bound to the L2 site is either slowly (within hours) or not convertible to Zx. 3) Vx bound to L1 (only in recombinant proteins) is not convertible to Zx.	bind
16914	9	6270	5	NULL	NULL	0	NULL	statement 8	NULL		is not convertible to	NULL				Zx	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_31_21924_s_233	16754673	1) Vx bound to the N1 and V1 site is rapidly (within 10-20 min) convertible to Zx. 2) Vx bound to the L2 site is either slowly (within hours) or not convertible to Zx. 3) Vx bound to L1 (only in recombinant proteins) is not convertible to Zx.	bind
21644	1	6270	7	NULL	NULL	NULL	NULL	 Vx	Chemical		bind								N1 site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_31_21924_s_233	16754673	1) Vx bound to the N1 and V1 site is rapidly (within 10-20 min) convertible to Zx. 2) Vx bound to the L2 site is either slowly (within hours) or not convertible to Zx. 3) Vx bound to L1 (only in recombinant proteins) is not convertible to Zx.	bind
21645	2	6270	7	NULL	NULL	NULL	NULL	Vx	Chemical		bind								V1 site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_31_21924_s_233	16754673	1) Vx bound to the N1 and V1 site is rapidly (within 10-20 min) convertible to Zx. 2) Vx bound to the L2 site is either slowly (within hours) or not convertible to Zx. 3) Vx bound to L1 (only in recombinant proteins) is not convertible to Zx.	bind
21646	3	6270	7	NULL	NULL	NULL	NULL	statement 1	Process		converts to		rapidly			Zx	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_31_21924_s_233	16754673	1) Vx bound to the N1 and V1 site is rapidly (within 10-20 min) convertible to Zx. 2) Vx bound to the L2 site is either slowly (within hours) or not convertible to Zx. 3) Vx bound to L1 (only in recombinant proteins) is not convertible to Zx.	bind
21647	4	6270	7	NULL	NULL	NULL	NULL	Vx	Chemical		binds to								L2 site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_31_21924_s_233	16754673	1) Vx bound to the N1 and V1 site is rapidly (within 10-20 min) convertible to Zx. 2) Vx bound to the L2 site is either slowly (within hours) or not convertible to Zx. 3) Vx bound to L1 (only in recombinant proteins) is not convertible to Zx.	bind
21648	5	6270	7	NULL	NULL	NULL	NULL	statement 4	Process		is not converted to					Zx	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_31_21924_s_233	16754673	1) Vx bound to the N1 and V1 site is rapidly (within 10-20 min) convertible to Zx. 2) Vx bound to the L2 site is either slowly (within hours) or not convertible to Zx. 3) Vx bound to L1 (only in recombinant proteins) is not convertible to Zx.	bind
21649	6	6270	7	NULL	NULL	NULL	NULL	Vx	Chemical		bind		only					recombinant	L1 		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_31_21924_s_233	16754673	1) Vx bound to the N1 and V1 site is rapidly (within 10-20 min) convertible to Zx. 2) Vx bound to the L2 site is either slowly (within hours) or not convertible to Zx. 3) Vx bound to L1 (only in recombinant proteins) is not convertible to Zx.	bind
21650	7	6270	7	NULL	NULL	NULL	NULL	statement 6	Process		is not converted to					Zx	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_31_21924_s_233	16754673	1) Vx bound to the N1 and V1 site is rapidly (within 10-20 min) convertible to Zx. 2) Vx bound to the L2 site is either slowly (within hours) or not convertible to Zx. 3) Vx bound to L1 (only in recombinant proteins) is not convertible to Zx.	bind
21651	8	6270	7	NULL	NULL	NULL	NULL	statement 4	Process		converts to		slowly			Zx	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_31_21924_s_233	16754673	1) Vx bound to the N1 and V1 site is rapidly (within 10-20 min) convertible to Zx. 2) Vx bound to the L2 site is either slowly (within hours) or not convertible to Zx. 3) Vx bound to L1 (only in recombinant proteins) is not convertible to Zx.	bind
16915	1	6271	5	NULL	NULL	0	NULL	tropomyosin	NULL		bind	NULL				actin filaments	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_14_7836_s_135	7713874	1) We have demonstrated that  tropomyosin and troponin are actually bound to the actin filaments at  motility assay conditions.	bind
16916	2	6271	5	NULL	NULL	0	NULL	troponin	NULL		bind	NULL				actin filaments	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_14_7836_s_135	7713874	1) We have demonstrated that  tropomyosin and troponin are actually bound to the actin filaments at  motility assay conditions.	bind
21652	1	6271	7	NULL	NULL	NULL	NULL	tropomyosin	GP		bind					actin filaments	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_14_7836_s_135	7713874	1) We have demonstrated that  tropomyosin and troponin are actually bound to the actin filaments at  motility assay conditions.	bind
21653	2	6271	7	NULL	NULL	NULL	NULL	troponin 	GP		bind					actin filaments	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_14_7836_s_135	7713874	1) We have demonstrated that  tropomyosin and troponin are actually bound to the actin filaments at  motility assay conditions.	bind
16917	1	6272	5	10	NULL	0	NULL	PEA3			interact with					AP1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31225_s_210	8537388	1), inducer of  c-myc  gene promoter ( PuF), CCAAT enhancer binding protein, a  regulator of cell growth and differentiation ( C/EBP), a  primary target of signal transduction induced by epidermal growth  factor, phorbol ester and serum ( PEA3), a transcription factor  that interacts with AP1 in the regulation of SV40 gene expression ( AP-4), activator of  c-fos  gene expression and  induced by  c-sis  and platelet derived growth factor ( SIF), a transcription factor that binds to human  immunodeficiency virus  tar  element and to the TATA box ( UBP1).	bind
16918	2	6272	5	10	NULL	0	NULL	SIF			bind					human immunodeficiency virus				tar element	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31225_s_210	8537388	1), inducer of  c-myc  gene promoter ( PuF), CCAAT enhancer binding protein, a  regulator of cell growth and differentiation ( C/EBP), a  primary target of signal transduction induced by epidermal growth  factor, phorbol ester and serum ( PEA3), a transcription factor  that interacts with AP1 in the regulation of SV40 gene expression ( AP-4), activator of  c-fos  gene expression and  induced by  c-sis  and platelet derived growth factor ( SIF), a transcription factor that binds to human  immunodeficiency virus  tar  element and to the TATA box ( UBP1).	bind
16919	3	6272	5	10	NULL	0	NULL	SIF			bind					UBP1				TATA box	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31225_s_210	8537388	1), inducer of  c-myc  gene promoter ( PuF), CCAAT enhancer binding protein, a  regulator of cell growth and differentiation ( C/EBP), a  primary target of signal transduction induced by epidermal growth  factor, phorbol ester and serum ( PEA3), a transcription factor  that interacts with AP1 in the regulation of SV40 gene expression ( AP-4), activator of  c-fos  gene expression and  induced by  c-sis  and platelet derived growth factor ( SIF), a transcription factor that binds to human  immunodeficiency virus  tar  element and to the TATA box ( UBP1).	bind
54176	4	6272	5	10	NULL	0	NULL	C/EBP			regulates					cell		growth of;;differentiation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31225_s_210	8537388	1), inducer of  c-myc  gene promoter ( PuF), CCAAT enhancer binding protein, a  regulator of cell growth and differentiation ( C/EBP), a  primary target of signal transduction induced by epidermal growth  factor, phorbol ester and serum ( PEA3), a transcription factor  that interacts with AP1 in the regulation of SV40 gene expression ( AP-4), activator of  c-fos  gene expression and  induced by  c-sis  and platelet derived growth factor ( SIF), a transcription factor that binds to human  immunodeficiency virus  tar  element and to the TATA box ( UBP1).	bind
54177	5	6272	5	10	NULL	0	NULL	PEA3			is					phorbol ester and serum					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31225_s_210	8537388	1), inducer of  c-myc  gene promoter ( PuF), CCAAT enhancer binding protein, a  regulator of cell growth and differentiation ( C/EBP), a  primary target of signal transduction induced by epidermal growth  factor, phorbol ester and serum ( PEA3), a transcription factor  that interacts with AP1 in the regulation of SV40 gene expression ( AP-4), activator of  c-fos  gene expression and  induced by  c-sis  and platelet derived growth factor ( SIF), a transcription factor that binds to human  immunodeficiency virus  tar  element and to the TATA box ( UBP1).	bind
54178	6	6272	5	10	NULL	0	NULL	PEA3			is a type of					transcription factor					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31225_s_210	8537388	1), inducer of  c-myc  gene promoter ( PuF), CCAAT enhancer binding protein, a  regulator of cell growth and differentiation ( C/EBP), a  primary target of signal transduction induced by epidermal growth  factor, phorbol ester and serum ( PEA3), a transcription factor  that interacts with AP1 in the regulation of SV40 gene expression ( AP-4), activator of  c-fos  gene expression and  induced by  c-sis  and platelet derived growth factor ( SIF), a transcription factor that binds to human  immunodeficiency virus  tar  element and to the TATA box ( UBP1).	bind
54179	7	6272	5	10	NULL	0	NULL	statement 1			plays a role in					SV40 gene		regulation of;;expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31225_s_210	8537388	1), inducer of  c-myc  gene promoter ( PuF), CCAAT enhancer binding protein, a  regulator of cell growth and differentiation ( C/EBP), a  primary target of signal transduction induced by epidermal growth  factor, phorbol ester and serum ( PEA3), a transcription factor  that interacts with AP1 in the regulation of SV40 gene expression ( AP-4), activator of  c-fos  gene expression and  induced by  c-sis  and platelet derived growth factor ( SIF), a transcription factor that binds to human  immunodeficiency virus  tar  element and to the TATA box ( UBP1).	bind
54180	8	6272	5	10	NULL	0	NULL	SIF			is					c-sis and platelet derived growth factor					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31225_s_210	8537388	1), inducer of  c-myc  gene promoter ( PuF), CCAAT enhancer binding protein, a  regulator of cell growth and differentiation ( C/EBP), a  primary target of signal transduction induced by epidermal growth  factor, phorbol ester and serum ( PEA3), a transcription factor  that interacts with AP1 in the regulation of SV40 gene expression ( AP-4), activator of  c-fos  gene expression and  induced by  c-sis  and platelet derived growth factor ( SIF), a transcription factor that binds to human  immunodeficiency virus  tar  element and to the TATA box ( UBP1).	bind
54181	9	6272	5	10	NULL	0	NULL	SIF			is a type of					transcription factor					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31225_s_210	8537388	1), inducer of  c-myc  gene promoter ( PuF), CCAAT enhancer binding protein, a  regulator of cell growth and differentiation ( C/EBP), a  primary target of signal transduction induced by epidermal growth  factor, phorbol ester and serum ( PEA3), a transcription factor  that interacts with AP1 in the regulation of SV40 gene expression ( AP-4), activator of  c-fos  gene expression and  induced by  c-sis  and platelet derived growth factor ( SIF), a transcription factor that binds to human  immunodeficiency virus  tar  element and to the TATA box ( UBP1).	bind
54182	10	6272	5	10	NULL	0	NULL	PuF			is an inducer of					c-myc gene				promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31225_s_210	8537388	1), inducer of  c-myc  gene promoter ( PuF), CCAAT enhancer binding protein, a  regulator of cell growth and differentiation ( C/EBP), a  primary target of signal transduction induced by epidermal growth  factor, phorbol ester and serum ( PEA3), a transcription factor  that interacts with AP1 in the regulation of SV40 gene expression ( AP-4), activator of  c-fos  gene expression and  induced by  c-sis  and platelet derived growth factor ( SIF), a transcription factor that binds to human  immunodeficiency virus  tar  element and to the TATA box ( UBP1).	bind
54183	11	6272	5	10	NULL	0	NULL	C/EBP			is					CCAAT enhancer binding protein					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31225_s_210	8537388	1), inducer of  c-myc  gene promoter ( PuF), CCAAT enhancer binding protein, a  regulator of cell growth and differentiation ( C/EBP), a  primary target of signal transduction induced by epidermal growth  factor, phorbol ester and serum ( PEA3), a transcription factor  that interacts with AP1 in the regulation of SV40 gene expression ( AP-4), activator of  c-fos  gene expression and  induced by  c-sis  and platelet derived growth factor ( SIF), a transcription factor that binds to human  immunodeficiency virus  tar  element and to the TATA box ( UBP1).	bind
21688	1	6272	7	NULL	NULL	NULL	NULL	PEA3	Chemical		interacts with									 AP1	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31225_s_210	8537388	1), inducer of  c-myc  gene promoter ( PuF), CCAAT enhancer binding protein, a  regulator of cell growth and differentiation ( C/EBP), a  primary target of signal transduction induced by epidermal growth  factor, phorbol ester and serum ( PEA3), a transcription factor  that interacts with AP1 in the regulation of SV40 gene expression ( AP-4), activator of  c-fos  gene expression and  induced by  c-sis  and platelet derived growth factor ( SIF), a transcription factor that binds to human  immunodeficiency virus  tar  element and to the TATA box ( UBP1).	bind
21690	2	6272	7	NULL	NULL	NULL	NULL	statement 1	Process		regulates					SV40	Organism	expression of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31225_s_210	8537388	1), inducer of  c-myc  gene promoter ( PuF), CCAAT enhancer binding protein, a  regulator of cell growth and differentiation ( C/EBP), a  primary target of signal transduction induced by epidermal growth  factor, phorbol ester and serum ( PEA3), a transcription factor  that interacts with AP1 in the regulation of SV40 gene expression ( AP-4), activator of  c-fos  gene expression and  induced by  c-sis  and platelet derived growth factor ( SIF), a transcription factor that binds to human  immunodeficiency virus  tar  element and to the TATA box ( UBP1).	bind
21703	3	6272	7	NULL	NULL	NULL	NULL	PuF	GP		is a inducer of					c-myc gene	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31225_s_210	8537388	1), inducer of  c-myc  gene promoter ( PuF), CCAAT enhancer binding protein, a  regulator of cell growth and differentiation ( C/EBP), a  primary target of signal transduction induced by epidermal growth  factor, phorbol ester and serum ( PEA3), a transcription factor  that interacts with AP1 in the regulation of SV40 gene expression ( AP-4), activator of  c-fos  gene expression and  induced by  c-sis  and platelet derived growth factor ( SIF), a transcription factor that binds to human  immunodeficiency virus  tar  element and to the TATA box ( UBP1).	bind
21705	4	6272	7	NULL	NULL	NULL	NULL	C/EBP	GP		regulates					cell 	Cell	growth of;; differentiation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31225_s_210	8537388	1), inducer of  c-myc  gene promoter ( PuF), CCAAT enhancer binding protein, a  regulator of cell growth and differentiation ( C/EBP), a  primary target of signal transduction induced by epidermal growth  factor, phorbol ester and serum ( PEA3), a transcription factor  that interacts with AP1 in the regulation of SV40 gene expression ( AP-4), activator of  c-fos  gene expression and  induced by  c-sis  and platelet derived growth factor ( SIF), a transcription factor that binds to human  immunodeficiency virus  tar  element and to the TATA box ( UBP1).	bind
21707	5	6272	7	NULL	NULL	NULL	NULL	C/EBP	GP		is					CCAAT enhancer binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31225_s_210	8537388	1), inducer of  c-myc  gene promoter ( PuF), CCAAT enhancer binding protein, a  regulator of cell growth and differentiation ( C/EBP), a  primary target of signal transduction induced by epidermal growth  factor, phorbol ester and serum ( PEA3), a transcription factor  that interacts with AP1 in the regulation of SV40 gene expression ( AP-4), activator of  c-fos  gene expression and  induced by  c-sis  and platelet derived growth factor ( SIF), a transcription factor that binds to human  immunodeficiency virus  tar  element and to the TATA box ( UBP1).	bind
21709	6	6272	7	NULL	NULL	NULL	NULL	SIF	GP		bind							human immunodeficiency virus		tar element	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31225_s_210	8537388	1), inducer of  c-myc  gene promoter ( PuF), CCAAT enhancer binding protein, a  regulator of cell growth and differentiation ( C/EBP), a  primary target of signal transduction induced by epidermal growth  factor, phorbol ester and serum ( PEA3), a transcription factor  that interacts with AP1 in the regulation of SV40 gene expression ( AP-4), activator of  c-fos  gene expression and  induced by  c-sis  and platelet derived growth factor ( SIF), a transcription factor that binds to human  immunodeficiency virus  tar  element and to the TATA box ( UBP1).	bind
21712	7	6272	7	NULL	NULL	NULL	NULL	SIF	GP		bind					UBP1	GP			TATA box	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31225_s_210	8537388	1), inducer of  c-myc  gene promoter ( PuF), CCAAT enhancer binding protein, a  regulator of cell growth and differentiation ( C/EBP), a  primary target of signal transduction induced by epidermal growth  factor, phorbol ester and serum ( PEA3), a transcription factor  that interacts with AP1 in the regulation of SV40 gene expression ( AP-4), activator of  c-fos  gene expression and  induced by  c-sis  and platelet derived growth factor ( SIF), a transcription factor that binds to human  immunodeficiency virus  tar  element and to the TATA box ( UBP1).	bind
21714	8	6272	7	NULL	NULL	NULL	NULL	PEA3	Chemical		is					phorbol ester and serum	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31225_s_210	8537388	1), inducer of  c-myc  gene promoter ( PuF), CCAAT enhancer binding protein, a  regulator of cell growth and differentiation ( C/EBP), a  primary target of signal transduction induced by epidermal growth  factor, phorbol ester and serum ( PEA3), a transcription factor  that interacts with AP1 in the regulation of SV40 gene expression ( AP-4), activator of  c-fos  gene expression and  induced by  c-sis  and platelet derived growth factor ( SIF), a transcription factor that binds to human  immunodeficiency virus  tar  element and to the TATA box ( UBP1).	bind
21715	9	6272	7	NULL	NULL	NULL	NULL	SIF	GP		is					c-sis and platelet derived growth factor 	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31225_s_210	8537388	1), inducer of  c-myc  gene promoter ( PuF), CCAAT enhancer binding protein, a  regulator of cell growth and differentiation ( C/EBP), a  primary target of signal transduction induced by epidermal growth  factor, phorbol ester and serum ( PEA3), a transcription factor  that interacts with AP1 in the regulation of SV40 gene expression ( AP-4), activator of  c-fos  gene expression and  induced by  c-sis  and platelet derived growth factor ( SIF), a transcription factor that binds to human  immunodeficiency virus  tar  element and to the TATA box ( UBP1).	bind
55044	10	6272	7	NULL	NULL	NULL	NULL	SIF	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31225_s_210	8537388	1), inducer of  c-myc  gene promoter ( PuF), CCAAT enhancer binding protein, a  regulator of cell growth and differentiation ( C/EBP), a  primary target of signal transduction induced by epidermal growth  factor, phorbol ester and serum ( PEA3), a transcription factor  that interacts with AP1 in the regulation of SV40 gene expression ( AP-4), activator of  c-fos  gene expression and  induced by  c-sis  and platelet derived growth factor ( SIF), a transcription factor that binds to human  immunodeficiency virus  tar  element and to the TATA box ( UBP1).	bind
55045	11	6272	7	NULL	NULL	NULL	NULL	 PEA3	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31225_s_210	8537388	1), inducer of  c-myc  gene promoter ( PuF), CCAAT enhancer binding protein, a  regulator of cell growth and differentiation ( C/EBP), a  primary target of signal transduction induced by epidermal growth  factor, phorbol ester and serum ( PEA3), a transcription factor  that interacts with AP1 in the regulation of SV40 gene expression ( AP-4), activator of  c-fos  gene expression and  induced by  c-sis  and platelet derived growth factor ( SIF), a transcription factor that binds to human  immunodeficiency virus  tar  element and to the TATA box ( UBP1).	bind
16920	1	6273	5	10	NULL	0	NULL	NK cells	NULL	fetal	bind	NULL				Qa1b tetramers	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-immunol_162_12_10358137_s_5	10358137	1+Ly-49- cell lysates  contain CD94 protein and that a significant proportion of fetal NK cells  are bound by Qa1b tetramers.	bind
21719	1	6273	7	NULL	NULL	NULL	NULL	NK cells	Cell	fetal	bind					Qa1b tetramers	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-immunol_162_12_10358137_s_5	10358137	1+Ly-49- cell lysates  contain CD94 protein and that a significant proportion of fetal NK cells  are bound by Qa1b tetramers.	bind
21721	2	6273	7	NULL	NULL	NULL	NULL	Ly-49- cell lysates	Cell		contain					CD94 protein	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-immunol_162_12_10358137_s_5	10358137	1+Ly-49- cell lysates  contain CD94 protein and that a significant proportion of fetal NK cells  are bound by Qa1b tetramers.	bind
16921	1	6274	5	10	NULL	0	NULL	thiazolidinediones	NULL		activate	NULL				PPARgamma	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_404_s_16	12615657	1, 2 The activation of PPARgamma with a ligand, such as a class of antidiabetic, insulin-sensitizing agents known as thiazolidinediones, 3 or eicosanoid derivatives, including 15-deoxy-delta12,14-prostaglandin J2 (15d-PGJ2), 4 results in its heterodimerization with the retinoid X receptor and the binding of their complex to the PPAR response element (PPRE) of target genes.	bind
16922	2	6274	5	10	NULL	0	NULL	15d-PGJ2	NULL		activate	NULL				PPARgamma	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_404_s_16	12615657	1, 2 The activation of PPARgamma with a ligand, such as a class of antidiabetic, insulin-sensitizing agents known as thiazolidinediones, 3 or eicosanoid derivatives, including 15-deoxy-delta12,14-prostaglandin J2 (15d-PGJ2), 4 results in its heterodimerization with the retinoid X receptor and the binding of their complex to the PPAR response element (PPRE) of target genes.	bind
16923	3	6274	5	NULL	NULL	0	NULL	15d-PGJ2	NULL		is	NULL				15-deoxy-delta12,14-prostaglandin J2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_404_s_16	12615657	1, 2 The activation of PPARgamma with a ligand, such as a class of antidiabetic, insulin-sensitizing agents known as thiazolidinediones, 3 or eicosanoid derivatives, including 15-deoxy-delta12,14-prostaglandin J2 (15d-PGJ2), 4 results in its heterodimerization with the retinoid X receptor and the binding of their complex to the PPAR response element (PPRE) of target genes.	bind
16924	4	6274	5	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_404_s_16	12615657	1, 2 The activation of PPARgamma with a ligand, such as a class of antidiabetic, insulin-sensitizing agents known as thiazolidinediones, 3 or eicosanoid derivatives, including 15-deoxy-delta12,14-prostaglandin J2 (15d-PGJ2), 4 results in its heterodimerization with the retinoid X receptor and the binding of their complex to the PPAR response element (PPRE) of target genes.	bind
16925	5	6274	5	NULL	NULL	0	NULL	statement 1	NULL		results in	NULL				retinoid X receptor	NULL	heterodimerization with			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_404_s_16	12615657	1, 2 The activation of PPARgamma with a ligand, such as a class of antidiabetic, insulin-sensitizing agents known as thiazolidinediones, 3 or eicosanoid derivatives, including 15-deoxy-delta12,14-prostaglandin J2 (15d-PGJ2), 4 results in its heterodimerization with the retinoid X receptor and the binding of their complex to the PPAR response element (PPRE) of target genes.	bind
16926	6	6274	5	NULL	NULL	0	NULL	statement 2	NULL		results in	NULL				retinoid X receptor	NULL	heterodimerization with			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_404_s_16	12615657	1, 2 The activation of PPARgamma with a ligand, such as a class of antidiabetic, insulin-sensitizing agents known as thiazolidinediones, 3 or eicosanoid derivatives, including 15-deoxy-delta12,14-prostaglandin J2 (15d-PGJ2), 4 results in its heterodimerization with the retinoid X receptor and the binding of their complex to the PPAR response element (PPRE) of target genes.	bind
16927	7	6274	5	NULL	NULL	0	NULL	statement 5	NULL		bind	NULL				target genes	NULL			PPRE	NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_404_s_16	12615657	1, 2 The activation of PPARgamma with a ligand, such as a class of antidiabetic, insulin-sensitizing agents known as thiazolidinediones, 3 or eicosanoid derivatives, including 15-deoxy-delta12,14-prostaglandin J2 (15d-PGJ2), 4 results in its heterodimerization with the retinoid X receptor and the binding of their complex to the PPAR response element (PPRE) of target genes.	bind
16928	8	6274	5	NULL	NULL	0	NULL	PPRE	NULL		is	NULL				PPAR response element	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_404_s_16	12615657	1, 2 The activation of PPARgamma with a ligand, such as a class of antidiabetic, insulin-sensitizing agents known as thiazolidinediones, 3 or eicosanoid derivatives, including 15-deoxy-delta12,14-prostaglandin J2 (15d-PGJ2), 4 results in its heterodimerization with the retinoid X receptor and the binding of their complex to the PPAR response element (PPRE) of target genes.	bind
16929	9	6274	5	NULL	NULL	0	NULL	statement 6	NULL		bind	NULL				target genes	NULL			PPRE	NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_404_s_16	12615657	1, 2 The activation of PPARgamma with a ligand, such as a class of antidiabetic, insulin-sensitizing agents known as thiazolidinediones, 3 or eicosanoid derivatives, including 15-deoxy-delta12,14-prostaglandin J2 (15d-PGJ2), 4 results in its heterodimerization with the retinoid X receptor and the binding of their complex to the PPAR response element (PPRE) of target genes.	bind
45578	10	6274	5	10	NULL	0	NULL	thiazolidinediones	NULL		are type of	NULL				insulin-sensitizing agent	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_404_s_16	12615657	1, 2 The activation of PPARgamma with a ligand, such as a class of antidiabetic, insulin-sensitizing agents known as thiazolidinediones, 3 or eicosanoid derivatives, including 15-deoxy-delta12,14-prostaglandin J2 (15d-PGJ2), 4 results in its heterodimerization with the retinoid X receptor and the binding of their complex to the PPAR response element (PPRE) of target genes.	bind
21739	1	6274	7	NULL	NULL	NULL	NULL	 antidiabetic ligand	Chemical		activates					PPARgamma	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_404_s_16	12615657	1, 2 The activation of PPARgamma with a ligand, such as a class of antidiabetic, insulin-sensitizing agents known as thiazolidinediones, 3 or eicosanoid derivatives, including 15-deoxy-delta12,14-prostaglandin J2 (15d-PGJ2), 4 results in its heterodimerization with the retinoid X receptor and the binding of their complex to the PPAR response element (PPRE) of target genes.	bind
21741	2	6274	7	NULL	NULL	NULL	NULL	thiazolidinediones	Chemical		activates					PPARgamma	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_404_s_16	12615657	1, 2 The activation of PPARgamma with a ligand, such as a class of antidiabetic, insulin-sensitizing agents known as thiazolidinediones, 3 or eicosanoid derivatives, including 15-deoxy-delta12,14-prostaglandin J2 (15d-PGJ2), 4 results in its heterodimerization with the retinoid X receptor and the binding of their complex to the PPAR response element (PPRE) of target genes.	bind
21742	3	6274	7	NULL	NULL	NULL	NULL	15d-PGJ2	Chemical		activates					PPARgamma	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_404_s_16	12615657	1, 2 The activation of PPARgamma with a ligand, such as a class of antidiabetic, insulin-sensitizing agents known as thiazolidinediones, 3 or eicosanoid derivatives, including 15-deoxy-delta12,14-prostaglandin J2 (15d-PGJ2), 4 results in its heterodimerization with the retinoid X receptor and the binding of their complex to the PPAR response element (PPRE) of target genes.	bind
21747	4	6274	7	NULL	NULL	NULL	NULL	PPARgamma	GP	ligand activated	heterodimerizes					retinoid X receptor 	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_404_s_16	12615657	1, 2 The activation of PPARgamma with a ligand, such as a class of antidiabetic, insulin-sensitizing agents known as thiazolidinediones, 3 or eicosanoid derivatives, including 15-deoxy-delta12,14-prostaglandin J2 (15d-PGJ2), 4 results in its heterodimerization with the retinoid X receptor and the binding of their complex to the PPAR response element (PPRE) of target genes.	bind
21750	5	6274	7	NULL	NULL	NULL	NULL	statement 1	Process		results in					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_404_s_16	12615657	1, 2 The activation of PPARgamma with a ligand, such as a class of antidiabetic, insulin-sensitizing agents known as thiazolidinediones, 3 or eicosanoid derivatives, including 15-deoxy-delta12,14-prostaglandin J2 (15d-PGJ2), 4 results in its heterodimerization with the retinoid X receptor and the binding of their complex to the PPAR response element (PPRE) of target genes.	bind
21753	6	6274	7	NULL	NULL	NULL	NULL	statement 2	Process		results in					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_404_s_16	12615657	1, 2 The activation of PPARgamma with a ligand, such as a class of antidiabetic, insulin-sensitizing agents known as thiazolidinediones, 3 or eicosanoid derivatives, including 15-deoxy-delta12,14-prostaglandin J2 (15d-PGJ2), 4 results in its heterodimerization with the retinoid X receptor and the binding of their complex to the PPAR response element (PPRE) of target genes.	bind
21757	7	6274	7	NULL	NULL	NULL	NULL	statement 3	Process		results in					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_404_s_16	12615657	1, 2 The activation of PPARgamma with a ligand, such as a class of antidiabetic, insulin-sensitizing agents known as thiazolidinediones, 3 or eicosanoid derivatives, including 15-deoxy-delta12,14-prostaglandin J2 (15d-PGJ2), 4 results in its heterodimerization with the retinoid X receptor and the binding of their complex to the PPAR response element (PPRE) of target genes.	bind
21760	8	6274	7	NULL	NULL	NULL	NULL	statement 4	Process		bind									PPRE	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_404_s_16	12615657	1, 2 The activation of PPARgamma with a ligand, such as a class of antidiabetic, insulin-sensitizing agents known as thiazolidinediones, 3 or eicosanoid derivatives, including 15-deoxy-delta12,14-prostaglandin J2 (15d-PGJ2), 4 results in its heterodimerization with the retinoid X receptor and the binding of their complex to the PPAR response element (PPRE) of target genes.	bind
21762	9	6274	7	NULL	NULL	NULL	NULL	15d-PGJ2	GP		is					15-deoxy-delta12,14-prostaglandin J2 	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_404_s_16	12615657	1, 2 The activation of PPARgamma with a ligand, such as a class of antidiabetic, insulin-sensitizing agents known as thiazolidinediones, 3 or eicosanoid derivatives, including 15-deoxy-delta12,14-prostaglandin J2 (15d-PGJ2), 4 results in its heterodimerization with the retinoid X receptor and the binding of their complex to the PPAR response element (PPRE) of target genes.	bind
21763	10	6274	7	NULL	NULL	NULL	NULL	PPRE	GP		is					PPAR response element	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_404_s_16	12615657	1, 2 The activation of PPARgamma with a ligand, such as a class of antidiabetic, insulin-sensitizing agents known as thiazolidinediones, 3 or eicosanoid derivatives, including 15-deoxy-delta12,14-prostaglandin J2 (15d-PGJ2), 4 results in its heterodimerization with the retinoid X receptor and the binding of their complex to the PPAR response element (PPRE) of target genes.	bind
16930	1	6275	5	NULL	NULL	0	NULL	cGKIalpha	NULL		interact with	NULL	specifically	amino terminus		myosin phosphatase	NULL		myosin-binding subunit		NULL		0	NULL	NULL	NULL	gw60_circulationres_90_10_1080_s_25	12039797	1, 2, 25 Recent experiments have shown that the amino terminus of cGKIalpha interacts specifically with the myosin-binding subunit of myosin phosphatase, 12 whereas the amino terminus of cGKIbeta interacts specifically with inositol 1,4,5-trisphosphate receptor - associated cGMP kinase substrate (IRAG), a cGKI substrate protein.	bind
16931	2	6275	5	10	NULL	0	NULL	cGKIbeta 			interact with		specifically	amino terminus		IRAG					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_10_1080_s_25	12039797	1, 2, 25 Recent experiments have shown that the amino terminus of cGKIalpha interacts specifically with the myosin-binding subunit of myosin phosphatase, 12 whereas the amino terminus of cGKIbeta interacts specifically with inositol 1,4,5-trisphosphate receptor - associated cGMP kinase substrate (IRAG), a cGKI substrate protein.	bind
16932	3	6275	5	NULL	NULL	0	NULL	IRAG	NULL		is	NULL				1,4,5-trisphosphate receptor - associated cGMP kinase substrate	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_10_1080_s_25	12039797	1, 2, 25 Recent experiments have shown that the amino terminus of cGKIalpha interacts specifically with the myosin-binding subunit of myosin phosphatase, 12 whereas the amino terminus of cGKIbeta interacts specifically with inositol 1,4,5-trisphosphate receptor - associated cGMP kinase substrate (IRAG), a cGKI substrate protein.	bind
26090	4	6275	5	NULL	NULL	0	NULL	IRAG	NULL		is a type of	NULL				cGKI substrate protein	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_10_1080_s_25	12039797	1, 2, 25 Recent experiments have shown that the amino terminus of cGKIalpha interacts specifically with the myosin-binding subunit of myosin phosphatase, 12 whereas the amino terminus of cGKIbeta interacts specifically with inositol 1,4,5-trisphosphate receptor - associated cGMP kinase substrate (IRAG), a cGKI substrate protein.	bind
21771	1	6275	7	NULL	NULL	NULL	NULL	cGKIalpha	GP		interacts		specifically	amino terminus		myosin phosphatase	GP		myosin-binding subunit 		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_10_1080_s_25	12039797	1, 2, 25 Recent experiments have shown that the amino terminus of cGKIalpha interacts specifically with the myosin-binding subunit of myosin phosphatase, 12 whereas the amino terminus of cGKIbeta interacts specifically with inositol 1,4,5-trisphosphate receptor - associated cGMP kinase substrate (IRAG), a cGKI substrate protein.	bind
21773	2	6275	7	NULL	NULL	NULL	NULL	cGKIbeta	GP		interacts		specifically	amino terminus		IRAG	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_10_1080_s_25	12039797	1, 2, 25 Recent experiments have shown that the amino terminus of cGKIalpha interacts specifically with the myosin-binding subunit of myosin phosphatase, 12 whereas the amino terminus of cGKIbeta interacts specifically with inositol 1,4,5-trisphosphate receptor - associated cGMP kinase substrate (IRAG), a cGKI substrate protein.	bind
21774	3	6275	7	NULL	NULL	NULL	NULL	IRAG	GP		is					inositol 1,4,5-trisphosphate receptor - associated cGMP kinase substrate	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_10_1080_s_25	12039797	1, 2, 25 Recent experiments have shown that the amino terminus of cGKIalpha interacts specifically with the myosin-binding subunit of myosin phosphatase, 12 whereas the amino terminus of cGKIbeta interacts specifically with inositol 1,4,5-trisphosphate receptor - associated cGMP kinase substrate (IRAG), a cGKI substrate protein.	bind
21775	4	6275	7	NULL	NULL	NULL	NULL	IRAG	GP		is a type of					cGKI substrate protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_10_1080_s_25	12039797	1, 2, 25 Recent experiments have shown that the amino terminus of cGKIalpha interacts specifically with the myosin-binding subunit of myosin phosphatase, 12 whereas the amino terminus of cGKIbeta interacts specifically with inositol 1,4,5-trisphosphate receptor - associated cGMP kinase substrate (IRAG), a cGKI substrate protein.	bind
16933	1	6276	5	NULL	NULL	0	NULL	CCR3	NULL		bind	NULL				eotaxin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_4_1195_s_25	10514402	1, 3  he chemokine receptor CCR3, which binds eotaxin, RANTES, monocyte chemotactic protein (MCP)-3, MCP-4, and some other chemokines, is expressed in human eosinophils, 4- 6  basophils, 7  and type 2 T helper (Th2) cells.	bind
16934	2	6276	5	NULL	NULL	0	NULL	CCR3	NULL		bind	NULL				RANTES	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_4_1195_s_25	10514402	1, 3  he chemokine receptor CCR3, which binds eotaxin, RANTES, monocyte chemotactic protein (MCP)-3, MCP-4, and some other chemokines, is expressed in human eosinophils, 4- 6  basophils, 7  and type 2 T helper (Th2) cells.	bind
16935	3	6276	5	10	NULL	0	NULL	CCR3	NULL		bind	NULL				(MCP)-3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_4_1195_s_25	10514402	1, 3  he chemokine receptor CCR3, which binds eotaxin, RANTES, monocyte chemotactic protein (MCP)-3, MCP-4, and some other chemokines, is expressed in human eosinophils, 4- 6  basophils, 7  and type 2 T helper (Th2) cells.	bind
16936	4	6276	5	NULL	NULL	0	NULL	CCR3	NULL		bind	NULL				MCP-4	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_4_1195_s_25	10514402	1, 3  he chemokine receptor CCR3, which binds eotaxin, RANTES, monocyte chemotactic protein (MCP)-3, MCP-4, and some other chemokines, is expressed in human eosinophils, 4- 6  basophils, 7  and type 2 T helper (Th2) cells.	bind
16937	5	6276	5	NULL	NULL	0	NULL	CCR3	NULL		bind	NULL				chemokines	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_4_1195_s_25	10514402	1, 3  he chemokine receptor CCR3, which binds eotaxin, RANTES, monocyte chemotactic protein (MCP)-3, MCP-4, and some other chemokines, is expressed in human eosinophils, 4- 6  basophils, 7  and type 2 T helper (Th2) cells.	bind
16938	6	6276	5	NULL	NULL	0	NULL	CCR3	NULL		is expressed in	NULL				eosinophils	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_4_1195_s_25	10514402	1, 3  he chemokine receptor CCR3, which binds eotaxin, RANTES, monocyte chemotactic protein (MCP)-3, MCP-4, and some other chemokines, is expressed in human eosinophils, 4- 6  basophils, 7  and type 2 T helper (Th2) cells.	bind
16939	7	6276	5	NULL	NULL	0	NULL	CCR3	NULL		is expressed in	NULL				basophils	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_4_1195_s_25	10514402	1, 3  he chemokine receptor CCR3, which binds eotaxin, RANTES, monocyte chemotactic protein (MCP)-3, MCP-4, and some other chemokines, is expressed in human eosinophils, 4- 6  basophils, 7  and type 2 T helper (Th2) cells.	bind
16940	8	6276	5	NULL	NULL	0	NULL	CCR3	NULL		is expressed in	NULL				Th2 cells	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_4_1195_s_25	10514402	1, 3  he chemokine receptor CCR3, which binds eotaxin, RANTES, monocyte chemotactic protein (MCP)-3, MCP-4, and some other chemokines, is expressed in human eosinophils, 4- 6  basophils, 7  and type 2 T helper (Th2) cells.	bind
16941	9	6276	5	NULL	NULL	0	NULL	Th2 cells	NULL		is	NULL				type 2 T helper cells	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_4_1195_s_25	10514402	1, 3  he chemokine receptor CCR3, which binds eotaxin, RANTES, monocyte chemotactic protein (MCP)-3, MCP-4, and some other chemokines, is expressed in human eosinophils, 4- 6  basophils, 7  and type 2 T helper (Th2) cells.	bind
26091	10	6276	5	NULL	NULL	0	NULL	CCR3	NULL		is a type of	NULL				chemokine receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_4_1195_s_25	10514402	1, 3  he chemokine receptor CCR3, which binds eotaxin, RANTES, monocyte chemotactic protein (MCP)-3, MCP-4, and some other chemokines, is expressed in human eosinophils, 4- 6  basophils, 7  and type 2 T helper (Th2) cells.	bind
45579	11	6276	5	10	NULL	0	NULL	MCP	NULL		is	NULL				monocyte chemotactic protein	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_4_1195_s_25	10514402	1, 3  he chemokine receptor CCR3, which binds eotaxin, RANTES, monocyte chemotactic protein (MCP)-3, MCP-4, and some other chemokines, is expressed in human eosinophils, 4- 6  basophils, 7  and type 2 T helper (Th2) cells.	bind
21776	1	6276	7	NULL	NULL	NULL	NULL	CCR3	GP		binds					eotaxin	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_4_1195_s_25	10514402	1, 3  he chemokine receptor CCR3, which binds eotaxin, RANTES, monocyte chemotactic protein (MCP)-3, MCP-4, and some other chemokines, is expressed in human eosinophils, 4- 6  basophils, 7  and type 2 T helper (Th2) cells.	bind
21777	2	6276	7	NULL	NULL	NULL	NULL	CCR3	GP		binds					RANTES	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_4_1195_s_25	10514402	1, 3  he chemokine receptor CCR3, which binds eotaxin, RANTES, monocyte chemotactic protein (MCP)-3, MCP-4, and some other chemokines, is expressed in human eosinophils, 4- 6  basophils, 7  and type 2 T helper (Th2) cells.	bind
21779	3	6276	7	NULL	NULL	NULL	NULL	CCR3	GP		binds					MCP-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_4_1195_s_25	10514402	1, 3  he chemokine receptor CCR3, which binds eotaxin, RANTES, monocyte chemotactic protein (MCP)-3, MCP-4, and some other chemokines, is expressed in human eosinophils, 4- 6  basophils, 7  and type 2 T helper (Th2) cells.	bind
21780	4	6276	7	NULL	NULL	NULL	NULL	CCR3	GP		binds					MCP-4	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_4_1195_s_25	10514402	1, 3  he chemokine receptor CCR3, which binds eotaxin, RANTES, monocyte chemotactic protein (MCP)-3, MCP-4, and some other chemokines, is expressed in human eosinophils, 4- 6  basophils, 7  and type 2 T helper (Th2) cells.	bind
21781	5	6276	7	NULL	NULL	NULL	NULL	CCR3	GP		is expressed in					 eosinophils	Cell	human			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_4_1195_s_25	10514402	1, 3  he chemokine receptor CCR3, which binds eotaxin, RANTES, monocyte chemotactic protein (MCP)-3, MCP-4, and some other chemokines, is expressed in human eosinophils, 4- 6  basophils, 7  and type 2 T helper (Th2) cells.	bind
21783	6	6276	7	NULL	NULL	NULL	NULL	CCR3	GP		is expressed in					basophils	Cell				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_4_1195_s_25	10514402	1, 3  he chemokine receptor CCR3, which binds eotaxin, RANTES, monocyte chemotactic protein (MCP)-3, MCP-4, and some other chemokines, is expressed in human eosinophils, 4- 6  basophils, 7  and type 2 T helper (Th2) cells.	bind
21785	7	6276	7	NULL	NULL	NULL	NULL	CCR3	GP		is expressed in					Th2 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_4_1195_s_25	10514402	1, 3  he chemokine receptor CCR3, which binds eotaxin, RANTES, monocyte chemotactic protein (MCP)-3, MCP-4, and some other chemokines, is expressed in human eosinophils, 4- 6  basophils, 7  and type 2 T helper (Th2) cells.	bind
21786	8	6276	7	NULL	NULL	NULL	NULL	MCP	GP		is					monocyte chemotactic protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_4_1195_s_25	10514402	1, 3  he chemokine receptor CCR3, which binds eotaxin, RANTES, monocyte chemotactic protein (MCP)-3, MCP-4, and some other chemokines, is expressed in human eosinophils, 4- 6  basophils, 7  and type 2 T helper (Th2) cells.	bind
21787	9	6276	7	NULL	NULL	NULL	NULL	Th2	Cell		is					type 2 T helper	Cell				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_4_1195_s_25	10514402	1, 3  he chemokine receptor CCR3, which binds eotaxin, RANTES, monocyte chemotactic protein (MCP)-3, MCP-4, and some other chemokines, is expressed in human eosinophils, 4- 6  basophils, 7  and type 2 T helper (Th2) cells.	bind
26376	10	6276	7	NULL	NULL	NULL	NULL	CCR3	GP		is a type of					chemokine receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_4_1195_s_25	10514402	1, 3  he chemokine receptor CCR3, which binds eotaxin, RANTES, monocyte chemotactic protein (MCP)-3, MCP-4, and some other chemokines, is expressed in human eosinophils, 4- 6  basophils, 7  and type 2 T helper (Th2) cells.	bind
26377	11	6276	7	NULL	NULL	NULL	NULL	CCR3	GP		bind					chemokines	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_4_1195_s_25	10514402	1, 3  he chemokine receptor CCR3, which binds eotaxin, RANTES, monocyte chemotactic protein (MCP)-3, MCP-4, and some other chemokines, is expressed in human eosinophils, 4- 6  basophils, 7  and type 2 T helper (Th2) cells.	bind
16942	1	6277	5	NULL	NULL	0	NULL	ORC	NULL	Drosophila	bind	NULL	specifically				NULL			ACE3	NULL		NULL	NULL	NULL	NULL	gw70_nature_430_6997_372_s_247	15254542	1, 8 13 (2002) |  ChemPort |            Austin, R. J., Orr-Weaver, T. L. & Bell, S. P.  Drosophila ORC specifically binds to ACE3, an origin of DNA replication control element.	bind
16943	2	6277	5	NULL	NULL	0	NULL	ACE3	NULL		is origin of	NULL					NULL			DNA replication control element	NULL		NULL	NULL	NULL	NULL	gw70_nature_430_6997_372_s_247	15254542	1, 8 13 (2002) |  ChemPort |            Austin, R. J., Orr-Weaver, T. L. & Bell, S. P.  Drosophila ORC specifically binds to ACE3, an origin of DNA replication control element.	bind
21792	1	6277	7	NULL	NULL	NULL	NULL	ORC	GP	Drosophila	binds		specifically							ACE3	NULL		NULL	NULL	NULL	NULL	gw70_nature_430_6997_372_s_247	15254542	1, 8 13 (2002) |  ChemPort |            Austin, R. J., Orr-Weaver, T. L. & Bell, S. P.  Drosophila ORC specifically binds to ACE3, an origin of DNA replication control element.	bind
21794	2	6277	7	NULL	NULL	NULL	NULL	ACE3	GP		is origin of									DNA replication control element	NULL		NULL	NULL	NULL	NULL	gw70_nature_430_6997_372_s_247	15254542	1, 8 13 (2002) |  ChemPort |            Austin, R. J., Orr-Weaver, T. L. & Bell, S. P.  Drosophila ORC specifically binds to ACE3, an origin of DNA replication control element.	bind
16944	1	6279	5	NULL	NULL	0	NULL	FLAG-Plk	NULL	WT	bind	NULL				GST-C	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_4_1984_s_138	11854496	1, FLAG-Plk WT protein bound to GST-C; 2, FLAG-deltaC1-401 protein bound to GST-C; 3, FLAG-deltaC1-401 protein (T210D) bound to GST-C.	bind
16945	2	6279	5	NULL	NULL	0	NULL	FLAG-deltaC1-401 protein	NULL		bind	NULL				GST-C	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_4_1984_s_138	11854496	1, FLAG-Plk WT protein bound to GST-C; 2, FLAG-deltaC1-401 protein bound to GST-C; 3, FLAG-deltaC1-401 protein (T210D) bound to GST-C.	bind
16946	3	6279	5	NULL	NULL	0	NULL	FLAG-deltaC1-401 protein	NULL		bind	NULL		T210D		GST-C	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_4_1984_s_138	11854496	1, FLAG-Plk WT protein bound to GST-C; 2, FLAG-deltaC1-401 protein bound to GST-C; 3, FLAG-deltaC1-401 protein (T210D) bound to GST-C.	bind
21801	1	6279	7	NULL	NULL	NULL	NULL	FLAG-Plk protein	GP	WT	bind					GST-C	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_4_1984_s_138	11854496	1, FLAG-Plk WT protein bound to GST-C; 2, FLAG-deltaC1-401 protein bound to GST-C; 3, FLAG-deltaC1-401 protein (T210D) bound to GST-C.	bind
21803	2	6279	7	NULL	NULL	NULL	NULL	FLAG-deltaC1-401 protein	GP		bind					GST-C	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_4_1984_s_138	11854496	1, FLAG-Plk WT protein bound to GST-C; 2, FLAG-deltaC1-401 protein bound to GST-C; 3, FLAG-deltaC1-401 protein (T210D) bound to GST-C.	bind
21804	3	6279	7	NULL	NULL	NULL	NULL	FLAG-deltaC1-401 protein	GP		bind			 T210D		GST-C	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_4_1984_s_138	11854496	1, FLAG-Plk WT protein bound to GST-C; 2, FLAG-deltaC1-401 protein bound to GST-C; 3, FLAG-deltaC1-401 protein (T210D) bound to GST-C.	bind
16947	1	6280	5	10	NULL	0	NULL	FPP	NULL		bind	NULL				FTase	NULL				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_303_1_1_s_41	12646157	1, FPP (blue) bound to FTase (PDB number 1FT2).	bind
21807	1	6280	7	NULL	NULL	NULL	NULL	FPP	Chemical		bind					FTase	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_303_1_1_s_41	12646157	1, FPP (blue) bound to FTase (PDB number 1FT2).	bind
16948	1	6281	5	NULL	NULL	0	NULL	Mex67p	NULL		bind	NULL				GST-Nup116p	NULL		repeats		NULL		0	NULL	NULL	NULL	gw60_cellbiol_150_4_695_s_227	10952996	1, Protein standard; 2, recombinant Mex67p/His-Mtr2p complex, expressed in  E.  coli, and purified by Ni-NTA affinity, FPLC-MonoS, and gel filtration chromatography; 3, Mex67p and Mtr2p bound to GST-Nup116p repeats.	bind
16949	2	6281	5	NULL	NULL	0	NULL	Mtr2p	NULL		bind	NULL				GST-Nup116p	NULL		repeats		NULL		0	NULL	NULL	NULL	gw60_cellbiol_150_4_695_s_227	10952996	1, Protein standard; 2, recombinant Mex67p/His-Mtr2p complex, expressed in  E.  coli, and purified by Ni-NTA affinity, FPLC-MonoS, and gel filtration chromatography; 3, Mex67p and Mtr2p bound to GST-Nup116p repeats.	bind
21808	1	6281	7	NULL	NULL	NULL	NULL	Mex67p	GP		bind					GST-Nup116p	GP		repeats		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_150_4_695_s_227	10952996	1, Protein standard; 2, recombinant Mex67p/His-Mtr2p complex, expressed in  E.  coli, and purified by Ni-NTA affinity, FPLC-MonoS, and gel filtration chromatography; 3, Mex67p and Mtr2p bound to GST-Nup116p repeats.	bind
21809	2	6281	7	NULL	NULL	NULL	NULL	Mtr2p	GP		bind					GST-Nup116p	GP		repeats		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_150_4_695_s_227	10952996	1, Protein standard; 2, recombinant Mex67p/His-Mtr2p complex, expressed in  E.  coli, and purified by Ni-NTA affinity, FPLC-MonoS, and gel filtration chromatography; 3, Mex67p and Mtr2p bound to GST-Nup116p repeats.	bind
16950	1	6282	5	NULL	NULL	0	NULL	R7.1	NULL		bind	NULL					NULL		alphaL I domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_12_10590_s_173	11781316	1, R7.1, and clone 38 bind to the alphaL I domain ( 8,  10,  28).	bind
21813	1	6282	7	NULL	NULL	NULL	NULL	R7.1	GP		bind								alphaL I domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10590_s_173	11781316	1, R7.1, and clone 38 bind to the alphaL I domain ( 8,  10,  28).	bind
16951	1	6283	5	NULL	NULL	0	NULL	Sox2 protein	NULL		bind	NULL	individually			DNA	NULL			enhancer	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_30_23387_s_345	10801796	1, Sox2 or Oct-3 proteins bound individually to the enhancer DNA are relatively inactive.	bind
16952	2	6283	5	NULL	NULL	0	NULL	Oct-3 protein	NULL		bind	NULL	individually			DNA	NULL			enhancer	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_30_23387_s_345	10801796	1, Sox2 or Oct-3 proteins bound individually to the enhancer DNA are relatively inactive.	bind
16953	3	6283	5	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_30_23387_s_345	10801796	1, Sox2 or Oct-3 proteins bound individually to the enhancer DNA are relatively inactive.	bind
16954	4	6283	5	NULL	NULL	0	NULL	statement 1	NULL		is	NULL				inactive	NULL	relatively			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_30_23387_s_345	10801796	1, Sox2 or Oct-3 proteins bound individually to the enhancer DNA are relatively inactive.	bind
16955	5	6283	5	NULL	NULL	0	NULL	statement 2	NULL		is	NULL				inactive	NULL	relatively			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_30_23387_s_345	10801796	1, Sox2 or Oct-3 proteins bound individually to the enhancer DNA are relatively inactive.	bind
21816	1	6283	7	NULL	NULL	NULL	NULL	 Sox2 protein	GP		bind					DNA	NucleicAcid			enhancer	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_30_23387_s_345	10801796	1, Sox2 or Oct-3 proteins bound individually to the enhancer DNA are relatively inactive.	bind
21817	2	6283	7	NULL	NULL	NULL	NULL	Oct-3 protein	GP		bind					DNA	NucleicAcid			enhancer	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_30_23387_s_345	10801796	1, Sox2 or Oct-3 proteins bound individually to the enhancer DNA are relatively inactive.	bind
21818	3	6283	7	NULL	NULL	NULL	NULL	statement 1	Process		is					inactive	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_30_23387_s_345	10801796	1, Sox2 or Oct-3 proteins bound individually to the enhancer DNA are relatively inactive.	bind
21819	4	6283	7	NULL	NULL	NULL	NULL	statement 2	Process		is					inactive	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_30_23387_s_345	10801796	1, Sox2 or Oct-3 proteins bound individually to the enhancer DNA are relatively inactive.	bind
54184	5	6283	7	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_30_23387_s_345	10801796	1, Sox2 or Oct-3 proteins bound individually to the enhancer DNA are relatively inactive.	bind
19287	1	6284	5	NULL	NULL	0	NULL	A52R	NULL		is	NULL				virally derived vaccinia protein	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
19288	2	6284	5	NULL	NULL	0	NULL	statement 1	NULL		acts as	NULL				dominant-negative form of MyD88	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
19289	3	6284	5	NULL	NULL	0	NULL	Yop proteins	NULL	Yersinia	interferes with	NULL				MAP3K	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
19290	4	6284	5	NULL	NULL	0	NULL	statement 3	NULL		prevents	NULL				IkappaBalpha	NULL	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
19291	5	6284	5	NULL	NULL	0	NULL	Yop proteins	NULL	Yersinia	interferes with	NULL				IKKbeta	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
19292	6	6284	5	NULL	NULL	0	NULL	statement 5	NULL		prevents	NULL				IkappaBalpha	NULL	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
19293	7	6284	5	NULL	NULL	0	NULL	UPEC virulence factors	NULL		interferes with	NULL				MAP kinase	NULL	activity of			NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
19294	8	6284	5	NULL	NULL	0	NULL	measles virus	NULL		prevents	NULL				IkappaBalpha	NULL	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
19295	9	6284	5	NULL	NULL	0	NULL	IkappaBalpha	NULL	phosphorylated	undergoes	NULL				ubiquitination	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
19296	10	6284	5	NULL	NULL	0	NULL	Vpu protein	NULL	Salmonella	inhibit	NULL				statement 9	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
19297	11	6284	5	NULL	NULL	0	NULL	Vpu protein	NULL	HIV-1	inhibit	NULL				statement 9	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
19298	12	6284	5	NULL	NULL	0	NULL	orthopoxviruses	NULL		dephosphorylate	NULL				IkappaBalpha	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
19299	13	6284	5	NULL	NULL	0	NULL	orthopoxviruses	NULL		inhibit	NULL				IkappaBalpha	NULL	degradation of phosphorylated			NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
19300	14	6284	5	NULL	NULL	0	NULL	ASFV-derived protein	NULL		acts as	NULL				IkappaB-like molecule	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
19301	15	6284	5	NULL	NULL	0	NULL	NF-kappaB	NULL		is translocated to	NULL				nucleus	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
19302	16	6284	5	NULL	NULL	0	NULL	statement 14	NULL		inhibit	NULL				statement 15	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
19303	17	6284	5	NULL	NULL	0	NULL	ZEBRA protein	NULL	EBV-derived	bind	NULL				p65	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
19304	18	6284	5	NULL	NULL	0	NULL	soluble toxin	NULL	M. ulcerans	prevent	NULL	may			p65	NULL	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
19305	19	6284	5	NULL	NULL	0	NULL	NF-kappaB	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
19306	20	6284	5	NULL	NULL	0	NULL	soluble toxin	NULL	M. ulcerans	prevent	NULL	may			statement 19	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
19307	21	6284	5	NULL	NULL	0	NULL	statement 18	NULL		is an alternative to	NULL				statement 20	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
19308	22	6284	5	NULL	NULL	0	NULL		NULL	T. gondii	prevents	NULL				NF-kappaB	NULL	nuclear translocation of 			NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
19309	23	6284	5	NULL	NULL	0	NULL		NULL	S. mansoni 	disrupt	NULL				statement 19	NULL				NULL	in nucleus	0	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
21883	1	6284	7	NULL	NULL	NULL	NULL	vaccinia protein	GP	virally derived 	acts as a			A52R		MyD88	GP	dominant-negative form of			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
21884	2	6284	7	NULL	NULL	NULL	NULL	Yop proteins	GP	Yersinia	interfere with					MAP3K	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
21885	3	6284	7	NULL	NULL	NULL	NULL	Yop proteins	GP	Yersinia	interfere with					IKKbeta	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
21886	4	6284	7	NULL	NULL	NULL	NULL	statement 2	Process		prevents					IkappaBalpha	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
21887	5	6284	7	NULL	NULL	NULL	NULL	statement 3	Process		prevents					IkappaBalpha	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
21888	7	6284	7	NULL	NULL	NULL	NULL	UPEC	GP	virulence factors	interfere with					MAP kinase	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
21889	6	6284	7	NULL	NULL	NULL	NULL	statement 2	Process		occur along with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
21890	8	6284	7	NULL	NULL	NULL	NULL	measles virus	Organism		prevents					IkappaBalpha	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
21891	9	6284	7	NULL	NULL	NULL	NULL	Vpu protein	GP	Salmonella 	inhibits					IkappaBalpha	GP	ubiquitination of;; phosphorylated 			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
21892	10	6284	7	NULL	NULL	NULL	NULL	HIV-1 Vpu protein	GP		inhibits					IkappaBalpha	GP	ubiquitination of;; phosphorylated 			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
21893	11	6284	7	NULL	NULL	NULL	NULL	orthopoxviruses	Organism		dephosphorylate					IkappaBalpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
21894	12	6284	7	NULL	NULL	NULL	NULL	orthopoxviruses	Organism		inhibit					phosphorylated protein	GP	degradation of			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
21895	13	6284	7	NULL	NULL	NULL	NULL	statement 11	Process		is an alternative to					statement 12	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
21896	14	6284	7	NULL	NULL	NULL	NULL	ASFV-derived protein 	GP		acts as an					IkappaB-like molecule 	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
21897	15	6284	7	NULL	NULL	NULL	NULL	statement 14	Process		inhibit					NF-kappaB 	GP	translocation to nucleus			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
21898	16	6284	7	NULL	NULL	NULL	NULL	ZEBRA protein 	GP	EBV-derived	binds to					p65	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
21899	17	6284	7	NULL	NULL	NULL	NULL	soluble toxin	GP	M. ulcerans	prevent		may			p65	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
21900	18	6284	7	NULL	NULL	NULL	NULL	NF-kappaB	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
21901	19	6284	7	NULL	NULL	NULL	NULL	soluble toxin	GP	M.ulcerans	prevent					statement 18	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
21902	20	6284	7	NULL	NULL	NULL	NULL	T. gondii	Organism		prevents					NF-kappaB	GP	nuclear translocation of			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
21903	21	6284	7	NULL	NULL	NULL	NULL	NF-kappaB	GP		bind					DNA	NucleicAcid				NULL	nucleus	NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
21904	22	6284	7	NULL	NULL	NULL	NULL	S. mansoni	Organism		disrupts					statement 21	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3311_s_36	12065467	1, virally derived vaccinia protein, A52R, acts as a dominant-negative form of MyD88; 2,  Yersinia Yop proteins interfere with MAP3K and IKKbeta to prevent phosphorylation of IkappaBalpha and UPEC virulence factors interfere with MAP kinase activity; 3, measles virus prevents phosphorylation of IkappaBalpha; 4,  Salmonella and HIV-1 Vpu protein inhibit ubiquitination of phosphorylated IkappaBalpha; 5, orthopoxviruses can either dephosphorylate IkappaBalpha or inhibit degradation of the phosphorylated protein; 6, an ASFV-derived protein acts as an IkappaB-like molecule to inhibit NF-kappaB translocation to the nucleus; 7, EBV-derived ZEBRA protein binds to p65; 8, soluble toxin from  M. ulcerans may prevent phosphorylation of p65 and/or binding of NF-kappaB to DNA; 9,  T. gondii prevents nuclear translocation of NF-kappaB; 10,  S. mansoni disrupts NF-kappaB binding to DNA in the nucleus.	bind
16956	1	6286	5	NULL	NULL	0	NULL	FGF2	NULL		bind	NULL				FGFRs	NULL	cell-surface			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_316_s_14	14684627	1,2  Binding of FGF2 to cell-surface tyrosine kinase FGF receptors (FGFRs) triggers receptor dimerization and autophosphorylation of tyrosine residues, which act as docking sites for downstream proteins leading to cell response.	bind
16957	2	6286	5	NULL	NULL	0	NULL	FGFRs	NULL		is	NULL				FGF receptors	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_316_s_14	14684627	1,2  Binding of FGF2 to cell-surface tyrosine kinase FGF receptors (FGFRs) triggers receptor dimerization and autophosphorylation of tyrosine residues, which act as docking sites for downstream proteins leading to cell response.	bind
16958	3	6286	5	NULL	NULL	0	NULL	statement 1	NULL		trigger	NULL				receptor dimerization	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_3_316_s_14	14684627	1,2  Binding of FGF2 to cell-surface tyrosine kinase FGF receptors (FGFRs) triggers receptor dimerization and autophosphorylation of tyrosine residues, which act as docking sites for downstream proteins leading to cell response.	bind
16959	4	6286	5	NULL	NULL	0	NULL	statement 1	NULL		trigger	NULL				autophosphorylation	NULL			tyrosine residues	NULL		0	NULL	NULL	NULL	gw70_circulationres_94_3_316_s_14	14684627	1,2  Binding of FGF2 to cell-surface tyrosine kinase FGF receptors (FGFRs) triggers receptor dimerization and autophosphorylation of tyrosine residues, which act as docking sites for downstream proteins leading to cell response.	bind
16960	5	6286	5	NULL	NULL	0	NULL	statement 4	NULL		act as	NULL				docking sites	NULL	for downstream proteins			NULL		0	NULL	NULL	NULL	gw70_circulationres_94_3_316_s_14	14684627	1,2  Binding of FGF2 to cell-surface tyrosine kinase FGF receptors (FGFRs) triggers receptor dimerization and autophosphorylation of tyrosine residues, which act as docking sites for downstream proteins leading to cell response.	bind
16961	6	6286	5	NULL	NULL	0	NULL	statement 5	NULL		leads to	NULL				cell response	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_3_316_s_14	14684627	1,2  Binding of FGF2 to cell-surface tyrosine kinase FGF receptors (FGFRs) triggers receptor dimerization and autophosphorylation of tyrosine residues, which act as docking sites for downstream proteins leading to cell response.	bind
21905	1	6286	7	NULL	NULL	NULL	NULL	FGF2	GP		bind					tyrosine kinase FGFRs	GP	cell-surface			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_316_s_14	14684627	1,2  Binding of FGF2 to cell-surface tyrosine kinase FGF receptors (FGFRs) triggers receptor dimerization and autophosphorylation of tyrosine residues, which act as docking sites for downstream proteins leading to cell response.	bind
21906	2	6286	7	NULL	NULL	NULL	NULL	statement 1	Process		triggers					receptor	GP	dimerzation of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_316_s_14	14684627	1,2  Binding of FGF2 to cell-surface tyrosine kinase FGF receptors (FGFRs) triggers receptor dimerization and autophosphorylation of tyrosine residues, which act as docking sites for downstream proteins leading to cell response.	bind
21908	3	6286	7	NULL	NULL	NULL	NULL	statement 1	Process		triggers					autophosphorylation	Process		tyrosine residues		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_316_s_14	14684627	1,2  Binding of FGF2 to cell-surface tyrosine kinase FGF receptors (FGFRs) triggers receptor dimerization and autophosphorylation of tyrosine residues, which act as docking sites for downstream proteins leading to cell response.	bind
21909	4	6286	7	NULL	NULL	NULL	NULL	statement 2	Process		occurs along with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_316_s_14	14684627	1,2  Binding of FGF2 to cell-surface tyrosine kinase FGF receptors (FGFRs) triggers receptor dimerization and autophosphorylation of tyrosine residues, which act as docking sites for downstream proteins leading to cell response.	bind
21910	5	6286	7	NULL	NULL	NULL	NULL	statement 4	Process		act as					downstream proteins	GP	docking site for			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_316_s_14	14684627	1,2  Binding of FGF2 to cell-surface tyrosine kinase FGF receptors (FGFRs) triggers receptor dimerization and autophosphorylation of tyrosine residues, which act as docking sites for downstream proteins leading to cell response.	bind
21911	6	6286	7	NULL	NULL	NULL	NULL	statement 5	Process		leads to					cell response	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_316_s_14	14684627	1,2  Binding of FGF2 to cell-surface tyrosine kinase FGF receptors (FGFRs) triggers receptor dimerization and autophosphorylation of tyrosine residues, which act as docking sites for downstream proteins leading to cell response.	bind
21914	7	6286	7	NULL	NULL	NULL	NULL	FGFRs	GP		is					FGF receptors	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_316_s_14	14684627	1,2  Binding of FGF2 to cell-surface tyrosine kinase FGF receptors (FGFRs) triggers receptor dimerization and autophosphorylation of tyrosine residues, which act as docking sites for downstream proteins leading to cell response.	bind
16962	1	6287	5	NULL	NULL	0	NULL	eIF4E	NULL		interact with	NULL				eIF4G	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_93_12_1218_s_225	14605021	1,2  eIF4E also interacts with eIF4G, a molecule that binds to other translation factors, including eIF4A and eIF3.	bind
16963	2	6287	5	NULL	NULL	0	NULL	eIF4G	NULL		bind	NULL				eIF4A	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_12_1218_s_225	14605021	1,2  eIF4E also interacts with eIF4G, a molecule that binds to other translation factors, including eIF4A and eIF3.	bind
16964	3	6287	5	NULL	NULL	0	NULL	eIF4G	NULL		bind	NULL				eIF3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_12_1218_s_225	14605021	1,2  eIF4E also interacts with eIF4G, a molecule that binds to other translation factors, including eIF4A and eIF3.	bind
26096	4	6287	5	NULL	NULL	0	NULL	eIF4A	NULL		is a type of	NULL				translation factor	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_93_12_1218_s_225	14605021	1,2  eIF4E also interacts with eIF4G, a molecule that binds to other translation factors, including eIF4A and eIF3.	bind
26097	5	6287	5	NULL	NULL	0	NULL	eIF3	NULL		is a type of	NULL				translation factor	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_93_12_1218_s_225	14605021	1,2  eIF4E also interacts with eIF4G, a molecule that binds to other translation factors, including eIF4A and eIF3.	bind
21915	1	6287	7	NULL	NULL	NULL	NULL	eIF4E	GP		interacts with					eIF4G	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_12_1218_s_225	14605021	1,2  eIF4E also interacts with eIF4G, a molecule that binds to other translation factors, including eIF4A and eIF3.	bind
21916	2	6287	7	NULL	NULL	NULL	NULL	eIF4G	GP		binds					eIF4A	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_12_1218_s_225	14605021	1,2  eIF4E also interacts with eIF4G, a molecule that binds to other translation factors, including eIF4A and eIF3.	bind
21917	3	6287	7	NULL	NULL	NULL	NULL	eIF4G	GP		binds					eIF3	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_12_1218_s_225	14605021	1,2  eIF4E also interacts with eIF4G, a molecule that binds to other translation factors, including eIF4A and eIF3.	bind
26378	4	6287	7	NULL	NULL	NULL	NULL	eIF4A	GP		is a type of					translation factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_12_1218_s_225	14605021	1,2  eIF4E also interacts with eIF4G, a molecule that binds to other translation factors, including eIF4A and eIF3.	bind
26379	5	6287	7	NULL	NULL	NULL	NULL	eIF3	GP		is a type of					translation factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_12_1218_s_225	14605021	1,2  eIF4E also interacts with eIF4G, a molecule that binds to other translation factors, including eIF4A and eIF3.	bind
16965	1	6288	5	NULL	NULL	0	NULL	eIF4E	NULL		bind	NULL				7-methylguanosine triphosphate ("`cap"`) structure	NULL			5''-end of cytoplasmic mRNA	NULL		0	NULL	NULL	NULL	gw70_circulationres_93_12_1218_s_19	14605021	1,2  eIF4E binds to the 7-methylguanosine triphosphate ("`cap"`) structure at the 5''-end of cytoplasmic mRNA and interacts with eIF4G, a large scaffold protein that binds to other translation factors, including eIF4A and eIF3.	bind
16966	2	6288	5	NULL	NULL	0	NULL	eIF4E	NULL		interacts with	NULL				eIF4G	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_12_1218_s_19	14605021	1,2  eIF4E binds to the 7-methylguanosine triphosphate ("`cap"`) structure at the 5''-end of cytoplasmic mRNA and interacts with eIF4G, a large scaffold protein that binds to other translation factors, including eIF4A and eIF3.	bind
16967	3	6288	5	NULL	NULL	0	NULL	eIF4G	NULL		bind	NULL				eIF4A	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_12_1218_s_19	14605021	1,2  eIF4E binds to the 7-methylguanosine triphosphate ("`cap"`) structure at the 5''-end of cytoplasmic mRNA and interacts with eIF4G, a large scaffold protein that binds to other translation factors, including eIF4A and eIF3.	bind
16968	4	6288	5	NULL	NULL	0	NULL	eIF4G	NULL		bind	NULL				eIF3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_12_1218_s_19	14605021	1,2  eIF4E binds to the 7-methylguanosine triphosphate ("`cap"`) structure at the 5''-end of cytoplasmic mRNA and interacts with eIF4G, a large scaffold protein that binds to other translation factors, including eIF4A and eIF3.	bind
26103	5	6288	5	NULL	NULL	0	NULL	eIF4G	NULL		is a type of	NULL				large scaffold protein	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_93_12_1218_s_19	14605021	1,2  eIF4E binds to the 7-methylguanosine triphosphate ("`cap"`) structure at the 5''-end of cytoplasmic mRNA and interacts with eIF4G, a large scaffold protein that binds to other translation factors, including eIF4A and eIF3.	bind
26104	6	6288	5	NULL	NULL	0	NULL	eIF4A	NULL		is a type of	NULL				translation factor	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_93_12_1218_s_19	14605021	1,2  eIF4E binds to the 7-methylguanosine triphosphate ("`cap"`) structure at the 5''-end of cytoplasmic mRNA and interacts with eIF4G, a large scaffold protein that binds to other translation factors, including eIF4A and eIF3.	bind
26106	7	6288	5	NULL	NULL	0	NULL	eIF3	NULL		is a type of	NULL				translation factor	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_93_12_1218_s_19	14605021	1,2  eIF4E binds to the 7-methylguanosine triphosphate ("`cap"`) structure at the 5''-end of cytoplasmic mRNA and interacts with eIF4G, a large scaffold protein that binds to other translation factors, including eIF4A and eIF3.	bind
21920	1	6288	7	NULL	NULL	NULL	NULL	eIF4E	GP		binds to					7-methylguanosine triphosphate	Chemical			5''-end of cytoplasmic mRNA	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_12_1218_s_19	14605021	1,2  eIF4E binds to the 7-methylguanosine triphosphate ("`cap"`) structure at the 5''-end of cytoplasmic mRNA and interacts with eIF4G, a large scaffold protein that binds to other translation factors, including eIF4A and eIF3.	bind
21930	2	6288	7	NULL	NULL	NULL	NULL	 eIF4E	GP		interact with					eIF4G	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_12_1218_s_19	14605021	1,2  eIF4E binds to the 7-methylguanosine triphosphate ("`cap"`) structure at the 5''-end of cytoplasmic mRNA and interacts with eIF4G, a large scaffold protein that binds to other translation factors, including eIF4A and eIF3.	bind
21931	3	6288	7	NULL	NULL	NULL	NULL	eIF4G	GP		bind					eIF4A	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_12_1218_s_19	14605021	1,2  eIF4E binds to the 7-methylguanosine triphosphate ("`cap"`) structure at the 5''-end of cytoplasmic mRNA and interacts with eIF4G, a large scaffold protein that binds to other translation factors, including eIF4A and eIF3.	bind
21932	4	6288	7	NULL	NULL	NULL	NULL	eIF4G	GP		bind					eIF3	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_12_1218_s_19	14605021	1,2  eIF4E binds to the 7-methylguanosine triphosphate ("`cap"`) structure at the 5''-end of cytoplasmic mRNA and interacts with eIF4G, a large scaffold protein that binds to other translation factors, including eIF4A and eIF3.	bind
26380	6	6288	7	NULL	NULL	NULL	NULL	eIF4G	GP		is a type of					scaffold protein	GP	large			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_12_1218_s_19	14605021	1,2  eIF4E binds to the 7-methylguanosine triphosphate ("`cap"`) structure at the 5''-end of cytoplasmic mRNA and interacts with eIF4G, a large scaffold protein that binds to other translation factors, including eIF4A and eIF3.	bind
26381	7	6288	7	NULL	NULL	NULL	NULL	eIF3	GP		is a type of					translation factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_12_1218_s_19	14605021	1,2  eIF4E binds to the 7-methylguanosine triphosphate ("`cap"`) structure at the 5''-end of cytoplasmic mRNA and interacts with eIF4G, a large scaffold protein that binds to other translation factors, including eIF4A and eIF3.	bind
26382	8	6288	7	NULL	NULL	NULL	NULL	 eIF4A	GP		is a type of					translation factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_12_1218_s_19	14605021	1,2  eIF4E binds to the 7-methylguanosine triphosphate ("`cap"`) structure at the 5''-end of cytoplasmic mRNA and interacts with eIF4G, a large scaffold protein that binds to other translation factors, including eIF4A and eIF3.	bind
16969	1	6289	5	10	NULL	0	NULL	heparin			bind					AT					NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1549_s_18	15231514	1,2  In 1973, Rosenberg and Damus suggested that heparin binds the protease inhibitor antithrombin (AT), causing a conformational change within AT, accelerating its reaction with the protease thrombin and the formation of an active complex between protease and inhibitor.	bind
16970	2	6289	5	NULL	NULL	0	NULL	AT	NULL		is	NULL				antithrombin	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1549_s_18	15231514	1,2  In 1973, Rosenberg and Damus suggested that heparin binds the protease inhibitor antithrombin (AT), causing a conformational change within AT, accelerating its reaction with the protease thrombin and the formation of an active complex between protease and inhibitor.	bind
16971	3	6289	5	10	NULL	0	NULL	statement 1	NULL		causes	NULL				AT	NULL	conformational change within			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1549_s_18	15231514	1,2  In 1973, Rosenberg and Damus suggested that heparin binds the protease inhibitor antithrombin (AT), causing a conformational change within AT, accelerating its reaction with the protease thrombin and the formation of an active complex between protease and inhibitor.	bind
16972	4	6289	5	10	NULL	0	NULL	statement 3			accelerate					statement 9					NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1549_s_18	15231514	1,2  In 1973, Rosenberg and Damus suggested that heparin binds the protease inhibitor antithrombin (AT), causing a conformational change within AT, accelerating its reaction with the protease thrombin and the formation of an active complex between protease and inhibitor.	bind
16973	5	6289	5	NULL	NULL	0	NULL	protease	NULL		forms complex with	NULL	active			inhibitor	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1549_s_18	15231514	1,2  In 1973, Rosenberg and Damus suggested that heparin binds the protease inhibitor antithrombin (AT), causing a conformational change within AT, accelerating its reaction with the protease thrombin and the formation of an active complex between protease and inhibitor.	bind
16974	6	6289	5	NULL	NULL	0	NULL	statement 3	NULL		accelerate	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1549_s_18	15231514	1,2  In 1973, Rosenberg and Damus suggested that heparin binds the protease inhibitor antithrombin (AT), causing a conformational change within AT, accelerating its reaction with the protease thrombin and the formation of an active complex between protease and inhibitor.	bind
54185	7	6289	5	10	NULL	0	NULL	antithrombin			is a type of					protease inhibitor					NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1549_s_18	15231514	1,2  In 1973, Rosenberg and Damus suggested that heparin binds the protease inhibitor antithrombin (AT), causing a conformational change within AT, accelerating its reaction with the protease thrombin and the formation of an active complex between protease and inhibitor.	bind
54187	8	6289	5	10	NULL	0	NULL	thrombin			is a type of					protease					NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1549_s_18	15231514	1,2  In 1973, Rosenberg and Damus suggested that heparin binds the protease inhibitor antithrombin (AT), causing a conformational change within AT, accelerating its reaction with the protease thrombin and the formation of an active complex between protease and inhibitor.	bind
54189	9	6289	5	10	NULL	0	NULL	AT			reacts with					thrombin					NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1549_s_18	15231514	1,2  In 1973, Rosenberg and Damus suggested that heparin binds the protease inhibitor antithrombin (AT), causing a conformational change within AT, accelerating its reaction with the protease thrombin and the formation of an active complex between protease and inhibitor.	bind
21938	1	6289	7	NULL	NULL	NULL	NULL	heparin	GP		binds					AT	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1549_s_18	15231514	1,2  In 1973, Rosenberg and Damus suggested that heparin binds the protease inhibitor antithrombin (AT), causing a conformational change within AT, accelerating its reaction with the protease thrombin and the formation of an active complex between protease and inhibitor.	bind
21940	2	6289	7	NULL	NULL	NULL	NULL	statement 1	Process		cause					AT	GP	conformational change within			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1549_s_18	15231514	1,2  In 1973, Rosenberg and Damus suggested that heparin binds the protease inhibitor antithrombin (AT), causing a conformational change within AT, accelerating its reaction with the protease thrombin and the formation of an active complex between protease and inhibitor.	bind
21941	3	6289	7	NULL	NULL	NULL	NULL	AT	GP		reacts with					thrombin	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1549_s_18	15231514	1,2  In 1973, Rosenberg and Damus suggested that heparin binds the protease inhibitor antithrombin (AT), causing a conformational change within AT, accelerating its reaction with the protease thrombin and the formation of an active complex between protease and inhibitor.	bind
21942	4	6289	7	NULL	NULL	NULL	NULL	statement 2	Process		accelerates					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1549_s_18	15231514	1,2  In 1973, Rosenberg and Damus suggested that heparin binds the protease inhibitor antithrombin (AT), causing a conformational change within AT, accelerating its reaction with the protease thrombin and the formation of an active complex between protease and inhibitor.	bind
21943	5	6289	7	NULL	NULL	NULL	NULL	protease	GP		complex with					inhibitor	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1549_s_18	15231514	1,2  In 1973, Rosenberg and Damus suggested that heparin binds the protease inhibitor antithrombin (AT), causing a conformational change within AT, accelerating its reaction with the protease thrombin and the formation of an active complex between protease and inhibitor.	bind
21944	6	6289	7	NULL	NULL	NULL	NULL	statement 2	Process		accelerates					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1549_s_18	15231514	1,2  In 1973, Rosenberg and Damus suggested that heparin binds the protease inhibitor antithrombin (AT), causing a conformational change within AT, accelerating its reaction with the protease thrombin and the formation of an active complex between protease and inhibitor.	bind
21945	7	6289	7	NULL	NULL	NULL	NULL	At	GP		is					antithrombin	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1549_s_18	15231514	1,2  In 1973, Rosenberg and Damus suggested that heparin binds the protease inhibitor antithrombin (AT), causing a conformational change within AT, accelerating its reaction with the protease thrombin and the formation of an active complex between protease and inhibitor.	bind
54186	8	6289	7	NULL	NULL	NULL	NULL	antithrombin	GP		is a type of					protease inhibitor	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1549_s_18	15231514	1,2  In 1973, Rosenberg and Damus suggested that heparin binds the protease inhibitor antithrombin (AT), causing a conformational change within AT, accelerating its reaction with the protease thrombin and the formation of an active complex between protease and inhibitor.	bind
54188	9	6289	7	NULL	NULL	NULL	NULL	thrombin	GP		is a type of					protease	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1549_s_18	15231514	1,2  In 1973, Rosenberg and Damus suggested that heparin binds the protease inhibitor antithrombin (AT), causing a conformational change within AT, accelerating its reaction with the protease thrombin and the formation of an active complex between protease and inhibitor.	bind
16975	1	6290	5	NULL	NULL	0	NULL	LXRalpha/RXRs heterodimers	NULL		bind	NULL					NULL			DR-4 - type sequence elements	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_3_622_s_16	15625283	1,2  LXRalpha/RXRs heterodimers bind to DR-4 - type sequence elements known as the LXR response element in their target genes.	bind
26111	2	6290	5	10	NULL	0	NULL	DR-4 - type sequence elements			is a type of									LXR response element	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_3_622_s_16	15625283	1,2  LXRalpha/RXRs heterodimers bind to DR-4 - type sequence elements known as the LXR response element in their target genes.	bind
21946	1	6290	7	NULL	NULL	NULL	NULL	LXRalpha/RXRs heterodimers	GP		binds to									DR-4 - type sequence elements	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_3_622_s_16	15625283	1,2  LXRalpha/RXRs heterodimers bind to DR-4 - type sequence elements known as the LXR response element in their target genes.	bind
21947	2	6290	7	NULL	NULL	NULL	NULL	DR-4 - type sequence elements	GP		is a type of									LXR response element	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_3_622_s_16	15625283	1,2  LXRalpha/RXRs heterodimers bind to DR-4 - type sequence elements known as the LXR response element in their target genes.	bind
16976	1	6291	5	NULL	NULL	0	NULL	versican core protein	NULL		bind	NULL		G1		HA	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_370_s_14	16385080	1,2  The amino-terminal globular domain (G1) of versican core protein binds to hyaluronan (HA) and affects cell adhesion, proliferation, and migration.	bind
16977	2	6291	5	NULL	NULL	0	NULL	HA	NULL		is	NULL				hyaluronan	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_3_370_s_14	16385080	1,2  The amino-terminal globular domain (G1) of versican core protein binds to hyaluronan (HA) and affects cell adhesion, proliferation, and migration.	bind
16978	3	6291	5	NULL	NULL	0	NULL	G1	NULL		is	NULL				amino-terminal globular domain	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_3_370_s_14	16385080	1,2  The amino-terminal globular domain (G1) of versican core protein binds to hyaluronan (HA) and affects cell adhesion, proliferation, and migration.	bind
16979	4	6291	5	NULL	NULL	0	NULL	statement 1	NULL		affect	NULL				cell adhesion	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_3_370_s_14	16385080	1,2  The amino-terminal globular domain (G1) of versican core protein binds to hyaluronan (HA) and affects cell adhesion, proliferation, and migration.	bind
16980	5	6291	5	NULL	NULL	0	NULL	statement 2	NULL		affect	NULL				proliferation	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_3_370_s_14	16385080	1,2  The amino-terminal globular domain (G1) of versican core protein binds to hyaluronan (HA) and affects cell adhesion, proliferation, and migration.	bind
16981	6	6291	5	NULL	NULL	0	NULL	statement 1	NULL		affect	NULL				migration	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_3_370_s_14	16385080	1,2  The amino-terminal globular domain (G1) of versican core protein binds to hyaluronan (HA) and affects cell adhesion, proliferation, and migration.	bind
21979	1	6291	7	NULL	NULL	NULL	NULL	versican core protein	GP		binds to			amino-terminal G1 domain		HA	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_370_s_14	16385080	1,2  The amino-terminal globular domain (G1) of versican core protein binds to hyaluronan (HA) and affects cell adhesion, proliferation, and migration.	bind
21980	2	6291	7	NULL	NULL	NULL	NULL	statement 1	Process		affects					cell adhesion	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_370_s_14	16385080	1,2  The amino-terminal globular domain (G1) of versican core protein binds to hyaluronan (HA) and affects cell adhesion, proliferation, and migration.	bind
21981	3	6291	7	NULL	NULL	NULL	NULL	statement 1	GP		affects					cell proliferation	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_370_s_14	16385080	1,2  The amino-terminal globular domain (G1) of versican core protein binds to hyaluronan (HA) and affects cell adhesion, proliferation, and migration.	bind
21982	4	6291	7	NULL	NULL	NULL	NULL	statement 1	GP		affects					cell migration	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_370_s_14	16385080	1,2  The amino-terminal globular domain (G1) of versican core protein binds to hyaluronan (HA) and affects cell adhesion, proliferation, and migration.	bind
21983	5	6291	7	NULL	NULL	NULL	NULL	G1	GP		is					globular domain	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_370_s_14	16385080	1,2  The amino-terminal globular domain (G1) of versican core protein binds to hyaluronan (HA) and affects cell adhesion, proliferation, and migration.	bind
21984	6	6291	7	NULL	NULL	NULL	NULL	HA	Chemical		is					hyaluronan	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_370_s_14	16385080	1,2  The amino-terminal globular domain (G1) of versican core protein binds to hyaluronan (HA) and affects cell adhesion, proliferation, and migration.	bind
16982	1	6292	5	NULL	NULL	0	NULL	biglycan proteoglycans	NULL	arterial	bind	NULL	avidly			apoB-containing lipoproteins	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2162_s_181	15345509	1,24,25   However, of particular relevance to this study are the recent observations that arterial biglycan proteoglycans avidly bind to apoB-containing and apoE-containing lipoproteins.	bind
16983	2	6292	5	NULL	NULL	0	NULL	biglycan proteoglycans	NULL	arterial	bind	NULL	avidly			apoE-containing lipoproteins	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2162_s_181	15345509	1,24,25   However, of particular relevance to this study are the recent observations that arterial biglycan proteoglycans avidly bind to apoB-containing and apoE-containing lipoproteins.	bind
21985	1	6292	7	NULL	NULL	NULL	NULL	biglycan proteoglycans	Chemical	arterial 	bind		avidly			apoB-containing lipoprotein	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2162_s_181	15345509	1,24,25   However, of particular relevance to this study are the recent observations that arterial biglycan proteoglycans avidly bind to apoB-containing and apoE-containing lipoproteins.	bind
21986	2	6292	7	NULL	NULL	NULL	NULL	biglycan proteoglycans	Chemical	arterial 	bind		avidly			apoE-containing lipoprotein	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2162_s_181	15345509	1,24,25   However, of particular relevance to this study are the recent observations that arterial biglycan proteoglycans avidly bind to apoB-containing and apoE-containing lipoproteins.	bind
16984	1	6293	5	10	NULL	0	NULL	1,25(OH)2D3			alters					EGFR membrane 		trafficking of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_41_38965_s_32	12181310	1,25(OH)2D3 alters EGFR membrane trafficking, down-regulates EGFR-growth signaling, and impairs binding of nuclear EGFR to cognate DNA sequences, which in turn decreases its transcriptional activity on the cyclin D1 promoter.	bind
16985	2	6293	5	NULL	NULL	0	NULL	1,25(OH)2D3	NULL		down-regulate	NULL				EGFR-growth signaling	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_41_38965_s_32	12181310	1,25(OH)2D3 alters EGFR membrane trafficking, down-regulates EGFR-growth signaling, and impairs binding of nuclear EGFR to cognate DNA sequences, which in turn decreases its transcriptional activity on the cyclin D1 promoter.	bind
16986	3	6293	5	NULL	NULL	0	NULL	EGFR	NULL	nuclear	bind	NULL				cognate DNA sequences	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_41_38965_s_32	12181310	1,25(OH)2D3 alters EGFR membrane trafficking, down-regulates EGFR-growth signaling, and impairs binding of nuclear EGFR to cognate DNA sequences, which in turn decreases its transcriptional activity on the cyclin D1 promoter.	bind
16987	4	6293	5	NULL	NULL	0	NULL	1,25(OH)2D3	NULL		impairs	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_41_38965_s_32	12181310	1,25(OH)2D3 alters EGFR membrane trafficking, down-regulates EGFR-growth signaling, and impairs binding of nuclear EGFR to cognate DNA sequences, which in turn decreases its transcriptional activity on the cyclin D1 promoter.	bind
16988	6	6293	5	NULL	NULL	0	NULL	statement 4	NULL		decrease	NULL				statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_41_38965_s_32	12181310	1,25(OH)2D3 alters EGFR membrane trafficking, down-regulates EGFR-growth signaling, and impairs binding of nuclear EGFR to cognate DNA sequences, which in turn decreases its transcriptional activity on the cyclin D1 promoter.	bind
16989	7	6293	5	NULL	NULL	0	NULL	statement 2	NULL		decrease	NULL				statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_41_38965_s_32	12181310	1,25(OH)2D3 alters EGFR membrane trafficking, down-regulates EGFR-growth signaling, and impairs binding of nuclear EGFR to cognate DNA sequences, which in turn decreases its transcriptional activity on the cyclin D1 promoter.	bind
16990	8	6293	5	NULL	NULL	0	NULL	statement 1	NULL		decrease	NULL				statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_41_38965_s_32	12181310	1,25(OH)2D3 alters EGFR membrane trafficking, down-regulates EGFR-growth signaling, and impairs binding of nuclear EGFR to cognate DNA sequences, which in turn decreases its transcriptional activity on the cyclin D1 promoter.	bind
26116	5	6293	5	NULL	NULL	0	NULL	1,25(OH)2D3	NULL		induces	NULL				cyclin D1	NULL	transcriptional activity of		promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_41_38965_s_32	12181310	1,25(OH)2D3 alters EGFR membrane trafficking, down-regulates EGFR-growth signaling, and impairs binding of nuclear EGFR to cognate DNA sequences, which in turn decreases its transcriptional activity on the cyclin D1 promoter.	bind
54201	9	6293	5	10	NULL	0	NULL	statement 4			decreases					cyclin D1		transcriptional activity of		promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_41_38965_s_32	12181310	1,25(OH)2D3 alters EGFR membrane trafficking, down-regulates EGFR-growth signaling, and impairs binding of nuclear EGFR to cognate DNA sequences, which in turn decreases its transcriptional activity on the cyclin D1 promoter.	bind
21987	1	6293	7	NULL	NULL	NULL	NULL	1,25(OH)2D3	Chemical		alters					 EGFR membrane	GP	trafficking of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_41_38965_s_32	12181310	1,25(OH)2D3 alters EGFR membrane trafficking, down-regulates EGFR-growth signaling, and impairs binding of nuclear EGFR to cognate DNA sequences, which in turn decreases its transcriptional activity on the cyclin D1 promoter.	bind
21988	2	6293	7	NULL	NULL	NULL	NULL	1,25(OH)2D3	Chemical		downregulates					EGFR-growth signaling	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_41_38965_s_32	12181310	1,25(OH)2D3 alters EGFR membrane trafficking, down-regulates EGFR-growth signaling, and impairs binding of nuclear EGFR to cognate DNA sequences, which in turn decreases its transcriptional activity on the cyclin D1 promoter.	bind
21989	3	6293	7	NULL	NULL	NULL	NULL	EGFR	GP	nuclear	binds					 cognate DNA sequences	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_41_38965_s_32	12181310	1,25(OH)2D3 alters EGFR membrane trafficking, down-regulates EGFR-growth signaling, and impairs binding of nuclear EGFR to cognate DNA sequences, which in turn decreases its transcriptional activity on the cyclin D1 promoter.	bind
21990	4	6293	7	NULL	NULL	NULL	NULL	1,25(OH)2D3	Chemical		impairs					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_41_38965_s_32	12181310	1,25(OH)2D3 alters EGFR membrane trafficking, down-regulates EGFR-growth signaling, and impairs binding of nuclear EGFR to cognate DNA sequences, which in turn decreases its transcriptional activity on the cyclin D1 promoter.	bind
21991	5	6293	7	NULL	NULL	NULL	NULL	statement 4	Process		decrease					cyclin D1	GP	transcriptional activity of		promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_41_38965_s_32	12181310	1,25(OH)2D3 alters EGFR membrane trafficking, down-regulates EGFR-growth signaling, and impairs binding of nuclear EGFR to cognate DNA sequences, which in turn decreases its transcriptional activity on the cyclin D1 promoter.	bind
26387	6	6293	7	NULL	NULL	NULL	NULL	1,25(OH)2D3	Process		induce					cyclin D1	GP	transcriptional activity of		promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_41_38965_s_32	12181310	1,25(OH)2D3 alters EGFR membrane trafficking, down-regulates EGFR-growth signaling, and impairs binding of nuclear EGFR to cognate DNA sequences, which in turn decreases its transcriptional activity on the cyclin D1 promoter.	bind
26388	7	6293	7	NULL	NULL	NULL	NULL	statement 1	Process		decrease					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_41_38965_s_32	12181310	1,25(OH)2D3 alters EGFR membrane trafficking, down-regulates EGFR-growth signaling, and impairs binding of nuclear EGFR to cognate DNA sequences, which in turn decreases its transcriptional activity on the cyclin D1 promoter.	bind
26389	8	6293	7	NULL	NULL	NULL	NULL	statement 2	Process		decrease					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_41_38965_s_32	12181310	1,25(OH)2D3 alters EGFR membrane trafficking, down-regulates EGFR-growth signaling, and impairs binding of nuclear EGFR to cognate DNA sequences, which in turn decreases its transcriptional activity on the cyclin D1 promoter.	bind
26390	9	6293	7	NULL	NULL	NULL	NULL	statement 4	Process		decrease					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_41_38965_s_32	12181310	1,25(OH)2D3 alters EGFR membrane trafficking, down-regulates EGFR-growth signaling, and impairs binding of nuclear EGFR to cognate DNA sequences, which in turn decreases its transcriptional activity on the cyclin D1 promoter.	bind
16991	1	6294	5	NULL	NULL	0	NULL	1,25-(OH)2-D3	NULL		repress	NULL				IL-2 gene	NULL	expression of			NULL	in T lymphocytes	NULL	NULL	NULL	NULL	gw60_febslett_436_3_329_s_8	9801142	1,25-(OH)2-D3 has also been shown to repress IL-2 gene expression in T lymphocytes by inhibiting complex formation between nuclear factor of activated T cells (NFATp) and AP-1 at the NFAT binding site of the IL-2 promoter.	bind
16993	3	6294	5	NULL	NULL	0	NULL	NFATp	NULL		is	NULL				nuclear factor of activated T cells	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_436_3_329_s_8	9801142	1,25-(OH)2-D3 has also been shown to repress IL-2 gene expression in T lymphocytes by inhibiting complex formation between nuclear factor of activated T cells (NFATp) and AP-1 at the NFAT binding site of the IL-2 promoter.	bind
16995	5	6294	5	NULL	NULL	0	NULL	NFATp	NULL		forms complex with	NULL				AP-1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_febslett_436_3_329_s_8	9801142	1,25-(OH)2-D3 has also been shown to repress IL-2 gene expression in T lymphocytes by inhibiting complex formation between nuclear factor of activated T cells (NFATp) and AP-1 at the NFAT binding site of the IL-2 promoter.	bind
16996	7	6294	5	NULL	NULL	0	NULL	statement 1	NULL		occurs by	NULL				statement 5	NULL	inhibiting			NULL		NULL	NULL	NULL	NULL	gw60_febslett_436_3_329_s_8	9801142	1,25-(OH)2-D3 has also been shown to repress IL-2 gene expression in T lymphocytes by inhibiting complex formation between nuclear factor of activated T cells (NFATp) and AP-1 at the NFAT binding site of the IL-2 promoter.	bind
26121	6	6294	5	NULL	NULL	0	NULL	statement 5	NULL		occurs at	NULL				NFAT binding site of the IL-2 promoter	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_436_3_329_s_8	9801142	1,25-(OH)2-D3 has also been shown to repress IL-2 gene expression in T lymphocytes by inhibiting complex formation between nuclear factor of activated T cells (NFATp) and AP-1 at the NFAT binding site of the IL-2 promoter.	bind
21992	1	6294	7	NULL	NULL	NULL	NULL	1,25-(OH)2-D3	GP		repress					 IL-2 gene	GP	expression of			NULL	T lymphocytes	NULL	NULL	NULL	NULL	gw60_febslett_436_3_329_s_8	9801142	1,25-(OH)2-D3 has also been shown to repress IL-2 gene expression in T lymphocytes by inhibiting complex formation between nuclear factor of activated T cells (NFATp) and AP-1 at the NFAT binding site of the IL-2 promoter.	bind
21993	2	6294	7	NULL	NULL	NULL	NULL	NFATp	GP		complex with					AP-1 	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_436_3_329_s_8	9801142	1,25-(OH)2-D3 has also been shown to repress IL-2 gene expression in T lymphocytes by inhibiting complex formation between nuclear factor of activated T cells (NFATp) and AP-1 at the NFAT binding site of the IL-2 promoter.	bind
21994	3	6294	7	NULL	NULL	NULL	NULL	1,25-(OH)2-D3	Chemical		inhibits					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_436_3_329_s_8	9801142	1,25-(OH)2-D3 has also been shown to repress IL-2 gene expression in T lymphocytes by inhibiting complex formation between nuclear factor of activated T cells (NFATp) and AP-1 at the NFAT binding site of the IL-2 promoter.	bind
21995	4	6294	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs upon					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_436_3_329_s_8	9801142	1,25-(OH)2-D3 has also been shown to repress IL-2 gene expression in T lymphocytes by inhibiting complex formation between nuclear factor of activated T cells (NFATp) and AP-1 at the NFAT binding site of the IL-2 promoter.	bind
21996	5	6294	7	NULL	NULL	NULL	NULL	NFATp	GP		is					nuclear factor of activated T cells	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_436_3_329_s_8	9801142	1,25-(OH)2-D3 has also been shown to repress IL-2 gene expression in T lymphocytes by inhibiting complex formation between nuclear factor of activated T cells (NFATp) and AP-1 at the NFAT binding site of the IL-2 promoter.	bind
26391	6	6294	7	NULL	NULL	NULL	NULL	statement 2	Process		occurs at					IL-2	GP			NFAT binding site promoter	NULL		NULL	NULL	NULL	NULL	gw60_febslett_436_3_329_s_8	9801142	1,25-(OH)2-D3 has also been shown to repress IL-2 gene expression in T lymphocytes by inhibiting complex formation between nuclear factor of activated T cells (NFATp) and AP-1 at the NFAT binding site of the IL-2 promoter.	bind
16997	1	6295	5	10	NULL	0	NULL	1,25-(OH)2D3			activates					VDR					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46862_s_16	12954644	1,25-(OH)2D3 activates the vitamin D receptor (VDR), a ligand-dependent transcription factor that binds  cis-acting DNA sequences known as vitamin D response elements ( ).	bind
16998	2	6295	5	NULL	NULL	0	NULL	VDR	NULL		is	NULL				vitamin D receptor	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46862_s_16	12954644	1,25-(OH)2D3 activates the vitamin D receptor (VDR), a ligand-dependent transcription factor that binds  cis-acting DNA sequences known as vitamin D response elements ( ).	bind
16999	3	6295	5	10	NULL	0	NULL	VDR			bind									vitamin D response elements	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46862_s_16	12954644	1,25-(OH)2D3 activates the vitamin D receptor (VDR), a ligand-dependent transcription factor that binds  cis-acting DNA sequences known as vitamin D response elements ( ).	bind
45580	4	6295	5	10	NULL	0	NULL	VDR			is a type of					ligand-dependent transcription factor					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46862_s_16	12954644	1,25-(OH)2D3 activates the vitamin D receptor (VDR), a ligand-dependent transcription factor that binds  cis-acting DNA sequences known as vitamin D response elements ( ).	bind
54202	5	6295	5	10	NULL	0	NULL	vitamin D response elements			is a type of					cis-acting DNA sequences					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46862_s_16	12954644	1,25-(OH)2D3 activates the vitamin D receptor (VDR), a ligand-dependent transcription factor that binds  cis-acting DNA sequences known as vitamin D response elements ( ).	bind
21997	1	6295	7	NULL	NULL	NULL	NULL	1,25-(OH)2D3	Chemical		activates					VDR	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46862_s_16	12954644	1,25-(OH)2D3 activates the vitamin D receptor (VDR), a ligand-dependent transcription factor that binds  cis-acting DNA sequences known as vitamin D response elements ( ).	bind
21998	2	6295	7	NULL	NULL	NULL	NULL	VDR	GP		binds									vitamin D response elements	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46862_s_16	12954644	1,25-(OH)2D3 activates the vitamin D receptor (VDR), a ligand-dependent transcription factor that binds  cis-acting DNA sequences known as vitamin D response elements ( ).	bind
21999	3	6295	7	NULL	NULL	NULL	NULL	VDR	GP		is a type of					ligand-dependent transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46862_s_16	12954644	1,25-(OH)2D3 activates the vitamin D receptor (VDR), a ligand-dependent transcription factor that binds  cis-acting DNA sequences known as vitamin D response elements ( ).	bind
22000	4	6295	7	NULL	NULL	NULL	NULL	VDR	GP		is					vitamin D receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46862_s_16	12954644	1,25-(OH)2D3 activates the vitamin D receptor (VDR), a ligand-dependent transcription factor that binds  cis-acting DNA sequences known as vitamin D response elements ( ).	bind
54203	5	6295	7	NULL	NULL	NULL	NULL	vitamin D response elements	GP		is a type of					cis-acting DNA sequences	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46862_s_16	12954644	1,25-(OH)2D3 activates the vitamin D receptor (VDR), a ligand-dependent transcription factor that binds  cis-acting DNA sequences known as vitamin D response elements ( ).	bind
17000	1	6296	5	NULL	NULL	0	NULL	OSF2	NULL		bind	NULL				OSE2	NULL				NULL	primary osteoblasts	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_1_110_s_155	8995235	1,25-(OH)2D3 Treatment of Primary Osteoblasts Abolishes Binding of OSF2 to OSE2	bind
17001	2	6296	5	10	NULL	0	NULL	1,25-(OH)2D3	NULL		abolishes	NULL				statement 1	NULL				NULL	primary osteoblasts	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_1_110_s_155	8995235	1,25-(OH)2D3 Treatment of Primary Osteoblasts Abolishes Binding of OSF2 to OSE2	bind
22002	1	6296	7	NULL	NULL	NULL	NULL	OSF2	GP		bind					OSE2	GP				NULL	primary osteoblast	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_1_110_s_155	8995235	1,25-(OH)2D3 Treatment of Primary Osteoblasts Abolishes Binding of OSF2 to OSE2	bind
22003	2	6296	7	NULL	NULL	NULL	NULL	1,25-(OH)2D3	Chemical		abolishes					statement 1	Process				NULL	Primary Osteoblasts	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_1_110_s_155	8995235	1,25-(OH)2D3 Treatment of Primary Osteoblasts Abolishes Binding of OSF2 to OSE2	bind
19196	1	6297	5	NULL	NULL	0	NULL	1,25-D3	NULL		induce	NULL				CYP3A4	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_60_6_1399_s_7	11723248	1,25-D3 uses the vitamin D receptor to induce CYP3A4 because a) the vitamin D receptor (VDR)-retinoid X receptor (RXR) heterodimer binds specifically to the  CYP3A4 ER6; b) selective mutation of the  CYP3A4 ER6 disrupted the binding of VDR-RXR; and c) reporter constructs containing only three copies of the CYP3A4 ER6 linked to a TK-CAT reporter were activated by 1,25-D3 only in cells cotransfected with a human VDR expression plasmid.	bind
19197	2	6297	5	NULL	NULL	0	NULL	1,25-D3	NULL		uses	NULL				vitamin D receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_60_6_1399_s_7	11723248	1,25-D3 uses the vitamin D receptor to induce CYP3A4 because a) the vitamin D receptor (VDR)-retinoid X receptor (RXR) heterodimer binds specifically to the  CYP3A4 ER6; b) selective mutation of the  CYP3A4 ER6 disrupted the binding of VDR-RXR; and c) reporter constructs containing only three copies of the CYP3A4 ER6 linked to a TK-CAT reporter were activated by 1,25-D3 only in cells cotransfected with a human VDR expression plasmid.	bind
19198	3	6297	5	NULL	NULL	0	NULL	statement 2	NULL		is required for	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_60_6_1399_s_7	11723248	1,25-D3 uses the vitamin D receptor to induce CYP3A4 because a) the vitamin D receptor (VDR)-retinoid X receptor (RXR) heterodimer binds specifically to the  CYP3A4 ER6; b) selective mutation of the  CYP3A4 ER6 disrupted the binding of VDR-RXR; and c) reporter constructs containing only three copies of the CYP3A4 ER6 linked to a TK-CAT reporter were activated by 1,25-D3 only in cells cotransfected with a human VDR expression plasmid.	bind
19200	4	6297	5	NULL	NULL	0	NULL	VDR-RXR heterodimer	NULL		is	NULL				vitamin D receptor-retinoid X receptor heterodimer	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_60_6_1399_s_7	11723248	1,25-D3 uses the vitamin D receptor to induce CYP3A4 because a) the vitamin D receptor (VDR)-retinoid X receptor (RXR) heterodimer binds specifically to the  CYP3A4 ER6; b) selective mutation of the  CYP3A4 ER6 disrupted the binding of VDR-RXR; and c) reporter constructs containing only three copies of the CYP3A4 ER6 linked to a TK-CAT reporter were activated by 1,25-D3 only in cells cotransfected with a human VDR expression plasmid.	bind
19205	5	6297	5	NULL	NULL	0	NULL	VDR-RXR heterodimer	NULL		bind	NULL	specifically			 CYP3A4	NULL			ER6	NULL		0	NULL	NULL	NULL	gw60_molpharmacol_60_6_1399_s_7	11723248	1,25-D3 uses the vitamin D receptor to induce CYP3A4 because a) the vitamin D receptor (VDR)-retinoid X receptor (RXR) heterodimer binds specifically to the  CYP3A4 ER6; b) selective mutation of the  CYP3A4 ER6 disrupted the binding of VDR-RXR; and c) reporter constructs containing only three copies of the CYP3A4 ER6 linked to a TK-CAT reporter were activated by 1,25-D3 only in cells cotransfected with a human VDR expression plasmid.	bind
19207	6	6297	5	NULL	NULL	0	NULL	CYP3A4	NULL	mutant	disrupt	NULL			ER6	VDR-RXR	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_60_6_1399_s_7	11723248	1,25-D3 uses the vitamin D receptor to induce CYP3A4 because a) the vitamin D receptor (VDR)-retinoid X receptor (RXR) heterodimer binds specifically to the  CYP3A4 ER6; b) selective mutation of the  CYP3A4 ER6 disrupted the binding of VDR-RXR; and c) reporter constructs containing only three copies of the CYP3A4 ER6 linked to a TK-CAT reporter were activated by 1,25-D3 only in cells cotransfected with a human VDR expression plasmid.	bind
19210	7	6297	5	NULL	NULL	0	NULL	1,25-D3	NULL		activate	NULL				CYP3A4	NULL			ER6	NULL	cells cotransfected with human VDR expression plasmid	NULL	NULL	NULL	NULL	gw60_molpharmacol_60_6_1399_s_7	11723248	1,25-D3 uses the vitamin D receptor to induce CYP3A4 because a) the vitamin D receptor (VDR)-retinoid X receptor (RXR) heterodimer binds specifically to the  CYP3A4 ER6; b) selective mutation of the  CYP3A4 ER6 disrupted the binding of VDR-RXR; and c) reporter constructs containing only three copies of the CYP3A4 ER6 linked to a TK-CAT reporter were activated by 1,25-D3 only in cells cotransfected with a human VDR expression plasmid.	bind
22004	1	6297	7	NULL	NULL	NULL	NULL	1,25-D3 	Chemical		use					vitamin D receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_60_6_1399_s_7	11723248	1,25-D3 uses the vitamin D receptor to induce CYP3A4 because a) the vitamin D receptor (VDR)-retinoid X receptor (RXR) heterodimer binds specifically to the  CYP3A4 ER6; b) selective mutation of the  CYP3A4 ER6 disrupted the binding of VDR-RXR; and c) reporter constructs containing only three copies of the CYP3A4 ER6 linked to a TK-CAT reporter were activated by 1,25-D3 only in cells cotransfected with a human VDR expression plasmid.	bind
22005	2	6297	7	NULL	NULL	NULL	NULL	statement 1	Process		induce					CYP3A4 	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_60_6_1399_s_7	11723248	1,25-D3 uses the vitamin D receptor to induce CYP3A4 because a) the vitamin D receptor (VDR)-retinoid X receptor (RXR) heterodimer binds specifically to the  CYP3A4 ER6; b) selective mutation of the  CYP3A4 ER6 disrupted the binding of VDR-RXR; and c) reporter constructs containing only three copies of the CYP3A4 ER6 linked to a TK-CAT reporter were activated by 1,25-D3 only in cells cotransfected with a human VDR expression plasmid.	bind
22006	3	6297	7	NULL	NULL	NULL	NULL	VDR/RXR heterodimer	GP		binds		specifically			CYP3A4	GP			 ER6	NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_60_6_1399_s_7	11723248	1,25-D3 uses the vitamin D receptor to induce CYP3A4 because a) the vitamin D receptor (VDR)-retinoid X receptor (RXR) heterodimer binds specifically to the  CYP3A4 ER6; b) selective mutation of the  CYP3A4 ER6 disrupted the binding of VDR-RXR; and c) reporter constructs containing only three copies of the CYP3A4 ER6 linked to a TK-CAT reporter were activated by 1,25-D3 only in cells cotransfected with a human VDR expression plasmid.	bind
22007	4	6297	7	NULL	NULL	NULL	NULL	VDR	GP		binds					RXR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_60_6_1399_s_7	11723248	1,25-D3 uses the vitamin D receptor to induce CYP3A4 because a) the vitamin D receptor (VDR)-retinoid X receptor (RXR) heterodimer binds specifically to the  CYP3A4 ER6; b) selective mutation of the  CYP3A4 ER6 disrupted the binding of VDR-RXR; and c) reporter constructs containing only three copies of the CYP3A4 ER6 linked to a TK-CAT reporter were activated by 1,25-D3 only in cells cotransfected with a human VDR expression plasmid.	bind
22008	5	6297	7	NULL	NULL	NULL	NULL	CYP3A4 	GP	mutation of	disrupts				ER6	statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_60_6_1399_s_7	11723248	1,25-D3 uses the vitamin D receptor to induce CYP3A4 because a) the vitamin D receptor (VDR)-retinoid X receptor (RXR) heterodimer binds specifically to the  CYP3A4 ER6; b) selective mutation of the  CYP3A4 ER6 disrupted the binding of VDR-RXR; and c) reporter constructs containing only three copies of the CYP3A4 ER6 linked to a TK-CAT reporter were activated by 1,25-D3 only in cells cotransfected with a human VDR expression plasmid.	bind
22009	6	6297	7	NULL	NULL	NULL	NULL	VDR	GP		is					vitamin D receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_60_6_1399_s_7	11723248	1,25-D3 uses the vitamin D receptor to induce CYP3A4 because a) the vitamin D receptor (VDR)-retinoid X receptor (RXR) heterodimer binds specifically to the  CYP3A4 ER6; b) selective mutation of the  CYP3A4 ER6 disrupted the binding of VDR-RXR; and c) reporter constructs containing only three copies of the CYP3A4 ER6 linked to a TK-CAT reporter were activated by 1,25-D3 only in cells cotransfected with a human VDR expression plasmid.	bind
22010	7	6297	7	NULL	NULL	NULL	NULL	RXR	GP		is					retinoid X receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_60_6_1399_s_7	11723248	1,25-D3 uses the vitamin D receptor to induce CYP3A4 because a) the vitamin D receptor (VDR)-retinoid X receptor (RXR) heterodimer binds specifically to the  CYP3A4 ER6; b) selective mutation of the  CYP3A4 ER6 disrupted the binding of VDR-RXR; and c) reporter constructs containing only three copies of the CYP3A4 ER6 linked to a TK-CAT reporter were activated by 1,25-D3 only in cells cotransfected with a human VDR expression plasmid.	bind
17002	1	6298	5	NULL	NULL	0	NULL	1,25-Dihydroxyvitamin D3	NULL		activates	NULL				PLD	NULL				NULL	Caco-2 cells	0	NULL	NULL	NULL	gw60_jbiolchem_271_36_21767_s_512	8702973	1,25-Dihydroxyvitamin D3 but not TPA activates PLD in Caco-2 cells via pp60c-src and RhoA.	bind
17003	2	6298	5	NULL	NULL	0	NULL	statement 1	NULL		via	NULL				pp60c-src	NULL				NULL	Caco-2 cells	0	NULL	NULL	NULL	gw60_jbiolchem_271_36_21767_s_512	8702973	1,25-Dihydroxyvitamin D3 but not TPA activates PLD in Caco-2 cells via pp60c-src and RhoA.	bind
17004	3	6298	5	NULL	NULL	0	NULL	statement 1	NULL		via	NULL				RhoA	NULL				NULL	Caco-2 cells	0	NULL	NULL	NULL	gw60_jbiolchem_271_36_21767_s_512	8702973	1,25-Dihydroxyvitamin D3 but not TPA activates PLD in Caco-2 cells via pp60c-src and RhoA.	bind
17005	4	6298	5	NULL	NULL	0	NULL	TPA	NULL		does not activate	NULL				PLD	NULL				NULL	Caco-2 cells	0	NULL	NULL	NULL	gw60_jbiolchem_271_36_21767_s_512	8702973	1,25-Dihydroxyvitamin D3 but not TPA activates PLD in Caco-2 cells via pp60c-src and RhoA.	bind
22011	1	6298	7	NULL	NULL	NULL	NULL	1,25-Dihydroxyvitamin D3	Chemical		activates					PLD	GP				NULL	Caco-2 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_36_21767_s_512	8702973	1,25-Dihydroxyvitamin D3 but not TPA activates PLD in Caco-2 cells via pp60c-src and RhoA.	bind
22012	2	6298	7	NULL	NULL	NULL	NULL	TPA	Chemical		does not activate					PLD	GP				NULL	Caco-2 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_36_21767_s_512	8702973	1,25-Dihydroxyvitamin D3 but not TPA activates PLD in Caco-2 cells via pp60c-src and RhoA.	bind
22013	3	6298	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs via					pp60c-src	Process				NULL	Caco-2 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_36_21767_s_512	8702973	1,25-Dihydroxyvitamin D3 but not TPA activates PLD in Caco-2 cells via pp60c-src and RhoA.	bind
22014	4	6298	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs via					RhoA	GP				NULL	Caco-2 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_36_21767_s_512	8702973	1,25-Dihydroxyvitamin D3 but not TPA activates PLD in Caco-2 cells via pp60c-src and RhoA.	bind
17006	1	6299	5	NULL	NULL	0	NULL	1,25-Dihydroxyvitamin D3	NULL		stimulate	NULL				Caco-2	NULL	differentiation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5073_s_606	9710591	1,25-Dihydroxyvitamin D3 Stimulates Activator Protein-1-dependent Caco-2 Cell Differentiation.	bind
17007	2	6299	5	NULL	NULL	0	NULL	Caco-2	NULL	differentiation of	depends on	NULL				activator protein-1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5073_s_606	9710591	1,25-Dihydroxyvitamin D3 Stimulates Activator Protein-1-dependent Caco-2 Cell Differentiation.	bind
22015	1	6299	7	NULL	NULL	NULL	NULL	Caco-2 Cells 	Cell	differentiation of	depends on					Activator Protein-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5073_s_606	9710591	1,25-Dihydroxyvitamin D3 Stimulates Activator Protein-1-dependent Caco-2 Cell Differentiation.	bind
22016	1	6299	7	NULL	NULL	NULL	NULL	1,25-Dihydroxyvitamin D3	Chemical		stimulates					Caco-2 cells	Cell	differentiation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5073_s_606	9710591	1,25-Dihydroxyvitamin D3 Stimulates Activator Protein-1-dependent Caco-2 Cell Differentiation.	bind
17008	1	6300	5	NULL	NULL	0	NULL	1,25-VD	NULL		inhibit	NULL				NF-kappaB	NULL	activity of			NULL	human lymphocytes	0	NULL	NULL	NULL	gw70_carcinogenesis_27_1_32_s_232	15987715	1,25-VD has been reported to inhibit NF-kappaB activity in human lymphocytes and fibroblasts by either decreasing NF-kappaB DNA binding capacity or decreasing the expression of its precursor protein ( , ).	bind
17009	2	6300	5	NULL	NULL	0	NULL	1,25-VD	NULL		inhibit	NULL				NF-kappaB	NULL	activity of			NULL	human fibroblasts	0	NULL	NULL	NULL	gw70_carcinogenesis_27_1_32_s_232	15987715	1,25-VD has been reported to inhibit NF-kappaB activity in human lymphocytes and fibroblasts by either decreasing NF-kappaB DNA binding capacity or decreasing the expression of its precursor protein ( , ).	bind
17010	4	6300	5	NULL	NULL	0	NULL	statement 1	NULL		occurs by	NULL				statement 3	NULL	decreasing			NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_1_32_s_232	15987715	1,25-VD has been reported to inhibit NF-kappaB activity in human lymphocytes and fibroblasts by either decreasing NF-kappaB DNA binding capacity or decreasing the expression of its precursor protein ( , ).	bind
17011	6	6300	5	NULL	NULL	0	NULL	statement 1	NULL		occurs by	NULL				statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_1_32_s_232	15987715	1,25-VD has been reported to inhibit NF-kappaB activity in human lymphocytes and fibroblasts by either decreasing NF-kappaB DNA binding capacity or decreasing the expression of its precursor protein ( , ).	bind
17012	7	6300	5	NULL	NULL	0	NULL	statement 4	NULL		is an alternative to	NULL				statement 6	NULL				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_1_32_s_232	15987715	1,25-VD has been reported to inhibit NF-kappaB activity in human lymphocytes and fibroblasts by either decreasing NF-kappaB DNA binding capacity or decreasing the expression of its precursor protein ( , ).	bind
17013	8	6300	5	NULL	NULL	0	NULL	statement 2	NULL		occurs by	NULL				statement 3	NULL	decreasing			NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_1_32_s_232	15987715	1,25-VD has been reported to inhibit NF-kappaB activity in human lymphocytes and fibroblasts by either decreasing NF-kappaB DNA binding capacity or decreasing the expression of its precursor protein ( , ).	bind
17014	9	6300	5	NULL	NULL	0	NULL	statement 2	NULL		occurs by	NULL				statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_1_32_s_232	15987715	1,25-VD has been reported to inhibit NF-kappaB activity in human lymphocytes and fibroblasts by either decreasing NF-kappaB DNA binding capacity or decreasing the expression of its precursor protein ( , ).	bind
17015	10	6300	5	NULL	NULL	0	NULL	statement 8	NULL		is an alternative to	NULL				statement 9	NULL				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_1_32_s_232	15987715	1,25-VD has been reported to inhibit NF-kappaB activity in human lymphocytes and fibroblasts by either decreasing NF-kappaB DNA binding capacity or decreasing the expression of its precursor protein ( , ).	bind
46194	3	6300	5	NULL	NULL	0	NULL	NF-kappaB	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_27_1_32_s_232	15987715	1,25-VD has been reported to inhibit NF-kappaB activity in human lymphocytes and fibroblasts by either decreasing NF-kappaB DNA binding capacity or decreasing the expression of its precursor protein ( , ).	bind
46196	5	6300	5	NULL	NULL	0	NULL	1,25-VD	NULL		decreases	NULL				NF-kappaB precursor protein	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_27_1_32_s_232	15987715	1,25-VD has been reported to inhibit NF-kappaB activity in human lymphocytes and fibroblasts by either decreasing NF-kappaB DNA binding capacity or decreasing the expression of its precursor protein ( , ).	bind
22017	1	6300	7	NULL	NULL	NULL	NULL	1,25-VD	Chemical		inhibits					NF-kappaB 	GP	activity of human			NULL	human lymphocytes	NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_1_32_s_232	15987715	1,25-VD has been reported to inhibit NF-kappaB activity in human lymphocytes and fibroblasts by either decreasing NF-kappaB DNA binding capacity or decreasing the expression of its precursor protein ( , ).	bind
22018	2	6300	7	NULL	NULL	NULL	NULL	1,25-VD	Chemical		inhibits					NF-kappaB	GP	activity of			NULL	fibroblasts	NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_1_32_s_232	15987715	1,25-VD has been reported to inhibit NF-kappaB activity in human lymphocytes and fibroblasts by either decreasing NF-kappaB DNA binding capacity or decreasing the expression of its precursor protein ( , ).	bind
22019	3	6300	7	NULL	NULL	NULL	NULL	NF-kappaB 	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_1_32_s_232	15987715	1,25-VD has been reported to inhibit NF-kappaB activity in human lymphocytes and fibroblasts by either decreasing NF-kappaB DNA binding capacity or decreasing the expression of its precursor protein ( , ).	bind
22020	4	6300	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs upon					statement 3	Process	decreasing			NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_1_32_s_232	15987715	1,25-VD has been reported to inhibit NF-kappaB activity in human lymphocytes and fibroblasts by either decreasing NF-kappaB DNA binding capacity or decreasing the expression of its precursor protein ( , ).	bind
22021	5	6300	7	NULL	NULL	NULL	NULL	statement 2	Process		occurs upon					statement 3	Process	decreasing			NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_1_32_s_232	15987715	1,25-VD has been reported to inhibit NF-kappaB activity in human lymphocytes and fibroblasts by either decreasing NF-kappaB DNA binding capacity or decreasing the expression of its precursor protein ( , ).	bind
22022	7	6300	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs upon					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_1_32_s_232	15987715	1,25-VD has been reported to inhibit NF-kappaB activity in human lymphocytes and fibroblasts by either decreasing NF-kappaB DNA binding capacity or decreasing the expression of its precursor protein ( , ).	bind
22023	6	6300	7	NULL	NULL	NULL	NULL	1,25-VD	Chemical		decrease					NF-kappaB	GP	expression of precursor protein			NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_1_32_s_232	15987715	1,25-VD has been reported to inhibit NF-kappaB activity in human lymphocytes and fibroblasts by either decreasing NF-kappaB DNA binding capacity or decreasing the expression of its precursor protein ( , ).	bind
22024	8	6300	7	NULL	NULL	NULL	NULL	statement 2	Process		occurs upon					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_1_32_s_232	15987715	1,25-VD has been reported to inhibit NF-kappaB activity in human lymphocytes and fibroblasts by either decreasing NF-kappaB DNA binding capacity or decreasing the expression of its precursor protein ( , ).	bind
22025	9	6300	7	NULL	NULL	NULL	NULL	statement 4	Process		is an alternative to					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_1_32_s_232	15987715	1,25-VD has been reported to inhibit NF-kappaB activity in human lymphocytes and fibroblasts by either decreasing NF-kappaB DNA binding capacity or decreasing the expression of its precursor protein ( , ).	bind
22026	10	6300	7	NULL	NULL	NULL	NULL	statement 5	Process		is an alternative to					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_1_32_s_232	15987715	1,25-VD has been reported to inhibit NF-kappaB activity in human lymphocytes and fibroblasts by either decreasing NF-kappaB DNA binding capacity or decreasing the expression of its precursor protein ( , ).	bind
19310	1	6301	5	10	NULL	0	NULL	1,25-VD			reduce					p50		levels of			NULL	human lymphocytes	NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_9_1883_s_257	16624828	1,25-VD has been shown to reduce levels of p50 and its precursor p105 and then decrease PMA-induced NF-kappaB binding to the IL-6promoter in human lymphocytes ( ).	bind
19311	2	6301	5	10	NULL	0	NULL	1,25-VD			reduce					p105		levels of			NULL	human lymphocytes	NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_9_1883_s_257	16624828	1,25-VD has been shown to reduce levels of p50 and its precursor p105 and then decrease PMA-induced NF-kappaB binding to the IL-6promoter in human lymphocytes ( ).	bind
19312	3	6301	5	NULL	NULL	0	NULL	p105	NULL		is a type of	NULL				precursor of p50	NULL				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_9_1883_s_257	16624828	1,25-VD has been shown to reduce levels of p50 and its precursor p105 and then decrease PMA-induced NF-kappaB binding to the IL-6promoter in human lymphocytes ( ).	bind
19313	4	6301	5	NULL	NULL	0	NULL	NF-kappaB	NULL		bind	NULL				IL-6	NULL			promoter	NULL	human lymphocytes	NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_9_1883_s_257	16624828	1,25-VD has been shown to reduce levels of p50 and its precursor p105 and then decrease PMA-induced NF-kappaB binding to the IL-6promoter in human lymphocytes ( ).	bind
19314	5	6301	5	NULL	NULL	0	NULL	PMA	NULL		induce	NULL				statement 4	NULL				NULL	human lymphocytes	0	NULL	NULL	NULL	gw70_carcinogenesis_27_9_1883_s_257	16624828	1,25-VD has been shown to reduce levels of p50 and its precursor p105 and then decrease PMA-induced NF-kappaB binding to the IL-6promoter in human lymphocytes ( ).	bind
19315	6	6301	5	NULL	NULL	0	NULL	1,25-VD	NULL		decrease	NULL				statement 5	NULL				NULL	human lymphocytes	NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_9_1883_s_257	16624828	1,25-VD has been shown to reduce levels of p50 and its precursor p105 and then decrease PMA-induced NF-kappaB binding to the IL-6promoter in human lymphocytes ( ).	bind
22027	1	6301	7	NULL	NULL	NULL	NULL	1,25-VD	Chemical		reduce					p50	GP	levels of			NULL	human lymphocytes	NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_9_1883_s_257	16624828	1,25-VD has been shown to reduce levels of p50 and its precursor p105 and then decrease PMA-induced NF-kappaB binding to the IL-6promoter in human lymphocytes ( ).	bind
22028	2	6301	7	NULL	NULL	NULL	NULL	1,25-VD	Chemical		reduce					p105	GP	levels of			NULL	human lymphocytes	NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_9_1883_s_257	16624828	1,25-VD has been shown to reduce levels of p50 and its precursor p105 and then decrease PMA-induced NF-kappaB binding to the IL-6promoter in human lymphocytes ( ).	bind
22029	3	6301	7	NULL	NULL	NULL	NULL	NF-kappaB	GP		bind					 IL-6	GP			promoter	NULL	human lymphocytes	NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_9_1883_s_257	16624828	1,25-VD has been shown to reduce levels of p50 and its precursor p105 and then decrease PMA-induced NF-kappaB binding to the IL-6promoter in human lymphocytes ( ).	bind
22030	4	6301	7	NULL	NULL	NULL	NULL	PMA	Chemical		induce					statement 3	Process				NULL	human lymphocytes	NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_9_1883_s_257	16624828	1,25-VD has been shown to reduce levels of p50 and its precursor p105 and then decrease PMA-induced NF-kappaB binding to the IL-6promoter in human lymphocytes ( ).	bind
22031	5	6301	7	NULL	NULL	NULL	NULL	1,25-VD	Chemical		decrease					statement 4	Process				NULL	human lymphocytes	NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_9_1883_s_257	16624828	1,25-VD has been shown to reduce levels of p50 and its precursor p105 and then decrease PMA-induced NF-kappaB binding to the IL-6promoter in human lymphocytes ( ).	bind
29273	6	6301	7	NULL	NULL	NULL	NULL	p105	GP		is a type of					p50 precursor	GP				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_9_1883_s_257	16624828	1,25-VD has been shown to reduce levels of p50 and its precursor p105 and then decrease PMA-induced NF-kappaB binding to the IL-6promoter in human lymphocytes ( ).	bind
19316	1	6303	5	NULL	NULL	0	NULL	1,3-Propanediol dehydrogenase	NULL		require	NULL				NAD(H)	NULL	as a cofactor			NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_154_2_337_s_139	9311132	1,3-Propanediol dehydrogenase requires NAD(H) as a cofactor, but the highly conserved NAD(H) binding fingerprint pattern G-X-G-X-X-G  [ 27] was not present in the amino acid sequence.	bind
19317	2	6303	5	NULL	NULL	0	NULL		NULL	highly conserved	is not present in	NULL		NAD(H) binding fingerprint pattern G-X-G-X-X-G		1,3-Propanediol dehydrogenase	NULL	amino acid sequence of			NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_154_2_337_s_139	9311132	1,3-Propanediol dehydrogenase requires NAD(H) as a cofactor, but the highly conserved NAD(H) binding fingerprint pattern G-X-G-X-X-G  [ 27] was not present in the amino acid sequence.	bind
46201	3	6303	5	NULL	NULL	0	NULL	NAD(H)	NULL		bind	NULL					NULL	highly conserved		fingerprint pattern G-X-G-X-X-G	NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_154_2_337_s_139	9311132	1,3-Propanediol dehydrogenase requires NAD(H) as a cofactor, but the highly conserved NAD(H) binding fingerprint pattern G-X-G-X-X-G  [ 27] was not present in the amino acid sequence.	bind
22032	1	6303	7	NULL	NULL	NULL	NULL	1,3-Propanediol dehydrogenase	GP		requires					NAD(H)	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_154_2_337_s_139	9311132	1,3-Propanediol dehydrogenase requires NAD(H) as a cofactor, but the highly conserved NAD(H) binding fingerprint pattern G-X-G-X-X-G  [ 27] was not present in the amino acid sequence.	bind
22033	2	6303	7	NULL	NULL	NULL	NULL	NAD(H) 	Chemical		bind							highly conserved	fingerprint pattern G-X-G-X-X-G		NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_154_2_337_s_139	9311132	1,3-Propanediol dehydrogenase requires NAD(H) as a cofactor, but the highly conserved NAD(H) binding fingerprint pattern G-X-G-X-X-G  [ 27] was not present in the amino acid sequence.	bind
29276	3	6303	7	NULL	NULL	NULL	NULL	NADH	Chemical		is not present in			fingerprint pattern G-X-G-X-X-G 		1,3-Propanediol dehydrogenase	GP	amino acid sequence of			NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_154_2_337_s_139	9311132	1,3-Propanediol dehydrogenase requires NAD(H) as a cofactor, but the highly conserved NAD(H) binding fingerprint pattern G-X-G-X-X-G  [ 27] was not present in the amino acid sequence.	bind
67932	4	6303	7	NULL	NULL	0	NULL	NADH	Chemical		is a type of					cofactor	Chemical				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_154_2_337_s_139	9311132	1,3-Propanediol dehydrogenase requires NAD(H) as a cofactor, but the highly conserved NAD(H) binding fingerprint pattern G-X-G-X-X-G  [ 27] was not present in the amino acid sequence.	bind
19318	1	6304	5	NULL	NULL	0	NULL	1,4 Angiotensin II	NULL		bind	NULL				G protein - coupled receptors	NULL				NULL	on the surface of cardiomyocytes	0	NULL	NULL	NULL	gw70_circulation_110_6_718_s_24	15289381	1,4  Angiotensin II and endothelin-1 bind to G protein - coupled receptors on the surface of cardiomyocytes.	bind
19319	2	6304	5	NULL	NULL	0	NULL	endothelin-1	NULL		bind	NULL				G protein - coupled receptors	NULL				NULL	on the surface of cardiomyocytes	0	NULL	NULL	NULL	gw70_circulation_110_6_718_s_24	15289381	1,4  Angiotensin II and endothelin-1 bind to G protein - coupled receptors on the surface of cardiomyocytes.	bind
22034	1	6304	7	NULL	NULL	NULL	NULL	1,4 Angiotensin II	GP		bind					G protein - coupled receptors 	GP				NULL	on the surface of cardiomyocytes	NULL	NULL	NULL	NULL	gw70_circulation_110_6_718_s_24	15289381	1,4  Angiotensin II and endothelin-1 bind to G protein - coupled receptors on the surface of cardiomyocytes.	bind
22035	2	6304	7	NULL	NULL	NULL	NULL	endothelin-1	GP		bind					G protein - coupled receptors 	GP				NULL	on the surface of cardiomyocytes	NULL	NULL	NULL	NULL	gw70_circulation_110_6_718_s_24	15289381	1,4  Angiotensin II and endothelin-1 bind to G protein - coupled receptors on the surface of cardiomyocytes.	bind
19320	1	6306	5	NULL	NULL	0	NULL	BRG-1	NULL		bind	NULL	preferentially			RXR	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1180_s_167	15774904	1,9,22   On the contrary, BRG-1 preferentially binds and activates zinc finger proteins (including RXR and RAR), whereas brm activates factors with 2 ankyrin repeat proteins.	bind
19321	2	6306	5	NULL	NULL	0	NULL	BRG-1	NULL		activates	NULL	preferentially			RXR	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1180_s_167	15774904	1,9,22   On the contrary, BRG-1 preferentially binds and activates zinc finger proteins (including RXR and RAR), whereas brm activates factors with 2 ankyrin repeat proteins.	bind
19322	3	6306	5	NULL	NULL	0	NULL	BRG-1	NULL		bind	NULL	preferentially			RAR	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1180_s_167	15774904	1,9,22   On the contrary, BRG-1 preferentially binds and activates zinc finger proteins (including RXR and RAR), whereas brm activates factors with 2 ankyrin repeat proteins.	bind
19323	4	6306	5	NULL	NULL	0	NULL	BRG-1	NULL		activates	NULL	preferentially			RAR	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1180_s_167	15774904	1,9,22   On the contrary, BRG-1 preferentially binds and activates zinc finger proteins (including RXR and RAR), whereas brm activates factors with 2 ankyrin repeat proteins.	bind
19324	5	6306	5	NULL	NULL	0	NULL	statement 1	NULL		occurs along with	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1180_s_167	15774904	1,9,22   On the contrary, BRG-1 preferentially binds and activates zinc finger proteins (including RXR and RAR), whereas brm activates factors with 2 ankyrin repeat proteins.	bind
19325	6	6306	5	NULL	NULL	0	NULL	brm	NULL		activates	NULL				factors with 2 ankyrin repeat proteins	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1180_s_167	15774904	1,9,22   On the contrary, BRG-1 preferentially binds and activates zinc finger proteins (including RXR and RAR), whereas brm activates factors with 2 ankyrin repeat proteins.	bind
45581	7	6306	5	10	NULL	0	NULL	RXR	NULL		is a type of	NULL				zinc finger protein	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1180_s_167	15774904	1,9,22   On the contrary, BRG-1 preferentially binds and activates zinc finger proteins (including RXR and RAR), whereas brm activates factors with 2 ankyrin repeat proteins.	bind
45582	8	6306	5	10	NULL	0	NULL	RAR	NULL		is a type of	NULL				zinc finger protein	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1180_s_167	15774904	1,9,22   On the contrary, BRG-1 preferentially binds and activates zinc finger proteins (including RXR and RAR), whereas brm activates factors with 2 ankyrin repeat proteins.	bind
46202	9	6306	5	NULL	NULL	0	NULL	statement 3	NULL		occurs along with	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1180_s_167	15774904	1,9,22   On the contrary, BRG-1 preferentially binds and activates zinc finger proteins (including RXR and RAR), whereas brm activates factors with 2 ankyrin repeat proteins.	bind
22036	1	6306	7	NULL	NULL	NULL	NULL	BRG-1	GP		binds		preferentially			RXR	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1180_s_167	15774904	1,9,22   On the contrary, BRG-1 preferentially binds and activates zinc finger proteins (including RXR and RAR), whereas brm activates factors with 2 ankyrin repeat proteins.	bind
22037	2	6306	7	NULL	NULL	NULL	NULL	BRG-1	GP		activates		preferentially			RXR	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1180_s_167	15774904	1,9,22   On the contrary, BRG-1 preferentially binds and activates zinc finger proteins (including RXR and RAR), whereas brm activates factors with 2 ankyrin repeat proteins.	bind
22038	3	6306	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs along with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1180_s_167	15774904	1,9,22   On the contrary, BRG-1 preferentially binds and activates zinc finger proteins (including RXR and RAR), whereas brm activates factors with 2 ankyrin repeat proteins.	bind
22039	4	6306	7	NULL	NULL	NULL	NULL	BRG-1	GP		binds		preferentially			RAR	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1180_s_167	15774904	1,9,22   On the contrary, BRG-1 preferentially binds and activates zinc finger proteins (including RXR and RAR), whereas brm activates factors with 2 ankyrin repeat proteins.	bind
22040	5	6306	7	NULL	NULL	NULL	NULL	BRG-1	GP		activates		preferentially			RAR	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1180_s_167	15774904	1,9,22   On the contrary, BRG-1 preferentially binds and activates zinc finger proteins (including RXR and RAR), whereas brm activates factors with 2 ankyrin repeat proteins.	bind
22041	6	6306	7	NULL	NULL	NULL	NULL	statement 4	Process		occurs along with					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1180_s_167	15774904	1,9,22   On the contrary, BRG-1 preferentially binds and activates zinc finger proteins (including RXR and RAR), whereas brm activates factors with 2 ankyrin repeat proteins.	bind
22042	7	6306	7	NULL	NULL	NULL	NULL	brm	GP		activates					factors with 2 ankyrin repeat proteins	GP		\\		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1180_s_167	15774904	1,9,22   On the contrary, BRG-1 preferentially binds and activates zinc finger proteins (including RXR and RAR), whereas brm activates factors with 2 ankyrin repeat proteins.	bind
45583	8	6306	7	NULL	NULL	NULL	NULL	RXR	GP		is a type of					zinc finger protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1180_s_167	15774904	1,9,22   On the contrary, BRG-1 preferentially binds and activates zinc finger proteins (including RXR and RAR), whereas brm activates factors with 2 ankyrin repeat proteins.	bind
45584	9	6306	7	NULL	NULL	NULL	NULL	RAR	GP		is a type of					zinc finger protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1180_s_167	15774904	1,9,22   On the contrary, BRG-1 preferentially binds and activates zinc finger proteins (including RXR and RAR), whereas brm activates factors with 2 ankyrin repeat proteins.	bind
19326	1	6308	5	NULL	NULL	0	NULL	RPA	NULL		bind	NULL				DNA	NULL	cisplatin-damaged			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_9_7476_s_72	12486030	1-4 and references therein), both RPA and XPC-hHR23B showed preferential binding to the cisplatin-damaged DNA over the nondamaged one, whereas the XPA-DNA interaction was observed only in the presence of excess amounts (Fig.  2 A).	bind
19327	2	6308	5	NULL	NULL	0	NULL	RPA	NULL		bind	NULL				DNA	NULL	undamaged			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_9_7476_s_72	12486030	1-4 and references therein), both RPA and XPC-hHR23B showed preferential binding to the cisplatin-damaged DNA over the nondamaged one, whereas the XPA-DNA interaction was observed only in the presence of excess amounts (Fig.  2 A).	bind
19328	3	6308	5	NULL	NULL	0	NULL	statement 1	NULL		is prefered over	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_9_7476_s_72	12486030	1-4 and references therein), both RPA and XPC-hHR23B showed preferential binding to the cisplatin-damaged DNA over the nondamaged one, whereas the XPA-DNA interaction was observed only in the presence of excess amounts (Fig.  2 A).	bind
19329	4	6308	5	NULL	NULL	0	NULL	XPC-hHR23B	NULL		bind	NULL				DNA	NULL	cisplatin-damaged			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_9_7476_s_72	12486030	1-4 and references therein), both RPA and XPC-hHR23B showed preferential binding to the cisplatin-damaged DNA over the nondamaged one, whereas the XPA-DNA interaction was observed only in the presence of excess amounts (Fig.  2 A).	bind
19330	5	6308	5	NULL	NULL	0	NULL	XPC-hHR23B	NULL		bind	NULL				DNA	NULL	undamaged			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_9_7476_s_72	12486030	1-4 and references therein), both RPA and XPC-hHR23B showed preferential binding to the cisplatin-damaged DNA over the nondamaged one, whereas the XPA-DNA interaction was observed only in the presence of excess amounts (Fig.  2 A).	bind
19331	6	6308	5	NULL	NULL	0	NULL	statement 4	NULL		is prefered over	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_9_7476_s_72	12486030	1-4 and references therein), both RPA and XPC-hHR23B showed preferential binding to the cisplatin-damaged DNA over the nondamaged one, whereas the XPA-DNA interaction was observed only in the presence of excess amounts (Fig.  2 A).	bind
19332	7	6308	5	NULL	NULL	0	NULL	XPA	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_9_7476_s_72	12486030	1-4 and references therein), both RPA and XPC-hHR23B showed preferential binding to the cisplatin-damaged DNA over the nondamaged one, whereas the XPA-DNA interaction was observed only in the presence of excess amounts (Fig.  2 A).	bind
22044	1	6308	7	NULL	NULL	NULL	NULL	 RPA	GP		binds		preferentially			DNA	NucleicAcid	cisplatin-damaged 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_7476_s_72	12486030	1-4 and references therein), both RPA and XPC-hHR23B showed preferential binding to the cisplatin-damaged DNA over the nondamaged one, whereas the XPA-DNA interaction was observed only in the presence of excess amounts (Fig.  2 A).	bind
22045	2	6308	7	NULL	NULL	NULL	NULL	RPA	GP		bind					DNA	NucleicAcid	non damaged 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_7476_s_72	12486030	1-4 and references therein), both RPA and XPC-hHR23B showed preferential binding to the cisplatin-damaged DNA over the nondamaged one, whereas the XPA-DNA interaction was observed only in the presence of excess amounts (Fig.  2 A).	bind
22046	3	6308	7	NULL	NULL	NULL	NULL	statement 1	Process		is preferred over					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_7476_s_72	12486030	1-4 and references therein), both RPA and XPC-hHR23B showed preferential binding to the cisplatin-damaged DNA over the nondamaged one, whereas the XPA-DNA interaction was observed only in the presence of excess amounts (Fig.  2 A).	bind
22047	4	6308	7	NULL	NULL	NULL	NULL	XPC-hHR23B	GP		binds		preferentially			DNA	NucleicAcid	cisplatin-damaged 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_7476_s_72	12486030	1-4 and references therein), both RPA and XPC-hHR23B showed preferential binding to the cisplatin-damaged DNA over the nondamaged one, whereas the XPA-DNA interaction was observed only in the presence of excess amounts (Fig.  2 A).	bind
22048	6	6308	7	NULL	NULL	NULL	NULL	statement 4	Process		is preferred over					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_7476_s_72	12486030	1-4 and references therein), both RPA and XPC-hHR23B showed preferential binding to the cisplatin-damaged DNA over the nondamaged one, whereas the XPA-DNA interaction was observed only in the presence of excess amounts (Fig.  2 A).	bind
29284	5	6308	7	NULL	NULL	NULL	NULL	XPC-hHR23B	GP		binds					DNA	NucleicAcid	nondamaged			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_7476_s_72	12486030	1-4 and references therein), both RPA and XPC-hHR23B showed preferential binding to the cisplatin-damaged DNA over the nondamaged one, whereas the XPA-DNA interaction was observed only in the presence of excess amounts (Fig.  2 A).	bind
29287	7	6308	7	NULL	NULL	NULL	NULL	XPA	GP		interacts with					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_7476_s_72	12486030	1-4 and references therein), both RPA and XPC-hHR23B showed preferential binding to the cisplatin-damaged DNA over the nondamaged one, whereas the XPA-DNA interaction was observed only in the presence of excess amounts (Fig.  2 A).	bind
19333	1	6310	5	NULL	NULL	0	NULL	1-alpha,25-dihydroxyvitamin D3	NULL		inhibit	NULL				lung cancer cell line	NULL	growth of			NULL		0	NULL	NULL	NULL	gw60_jclininvest_103_12_1729_s_250	10377179	1-alpha,25-dihydroxyvitamin D3 and all-trans retinoic acid inhibit the growth of a lung cancer cell line.	bind
19334	2	6310	5	NULL	NULL	0	NULL	trans retinoic acid	NULL		inhibit	NULL				lung cancer cell line	NULL	growth of			NULL		0	NULL	NULL	NULL	gw60_jclininvest_103_12_1729_s_250	10377179	1-alpha,25-dihydroxyvitamin D3 and all-trans retinoic acid inhibit the growth of a lung cancer cell line.	bind
22049	1	6310	7	NULL	NULL	NULL	NULL	1-alpha,25-dihydroxyvitamin D3	Chemical		inhibit					lung cancer cell line	Cell	growth of 			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_103_12_1729_s_250	10377179	1-alpha,25-dihydroxyvitamin D3 and all-trans retinoic acid inhibit the growth of a lung cancer cell line.	bind
22050	2	6310	7	NULL	NULL	NULL	NULL	all-trans retinoic acid	Chemical		inhibit					lung cancer cell line	Cell	growth of			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_103_12_1729_s_250	10377179	1-alpha,25-dihydroxyvitamin D3 and all-trans retinoic acid inhibit the growth of a lung cancer cell line.	bind
19377	1	6311	5	NULL	NULL	0	NULL	m-CPP	NULL		interacts with	NULL				neurotransmitter receptors	NULL				NULL	human brain	0	NULL	NULL	NULL	gw60_neuropharmacology_42_2_162_s_236	11804612	1-m-(chlorophenyl)piperazine (m-CPP) interactions with neurotransmitter receptors in the human brain.	bind
19378	2	6311	5	NULL	NULL	0	NULL	m-CPP	NULL		is	NULL				1-m-(chlorophenyl)piperazine	NULL				NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_42_2_162_s_236	11804612	1-m-(chlorophenyl)piperazine (m-CPP) interactions with neurotransmitter receptors in the human brain.	bind
22051	1	6311	7	NULL	NULL	NULL	NULL	m-CPP	Chemical		interacts with					neurotransmitter receptors	GP				NULL	human brain	NULL	NULL	NULL	NULL	gw60_neuropharmacology_42_2_162_s_236	11804612	1-m-(chlorophenyl)piperazine (m-CPP) interactions with neurotransmitter receptors in the human brain.	bind
22052	2	6311	7	NULL	NULL	NULL	NULL	m-CPP	Chemical		is					1-m-(chlorophenyl)piperazine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_42_2_162_s_236	11804612	1-m-(chlorophenyl)piperazine (m-CPP) interactions with neurotransmitter receptors in the human brain.	bind
19379	1	6312	5	10	NULL	0	NULL	PX-12			bind								Cys73 residue		NULL		NULL	NULL	NULL	NULL	gw70_annurevnutr_25_0_261_s_383	16011468	1-Methyl-propyl-2-imidazolozyl disulfide (PX-12), a TRX-1  inhibitor binding to the Cys73 residue, not only significantly potentiated the inhibitory  effect of cisplatin on pancreatic cancer ( 8) but also exhibited promising antitumor activities among a variety of tumor cell  lines both in vitro and in vivo ( 158).	bind
19380	2	6312	5	NULL	NULL	0	NULL	PX-12	NULL		is	NULL				1-Methyl-propyl-2-imidazolozyl disulfide	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevnutr_25_0_261_s_383	16011468	1-Methyl-propyl-2-imidazolozyl disulfide (PX-12), a TRX-1  inhibitor binding to the Cys73 residue, not only significantly potentiated the inhibitory  effect of cisplatin on pancreatic cancer ( 8) but also exhibited promising antitumor activities among a variety of tumor cell  lines both in vitro and in vivo ( 158).	bind
19381	3	6312	5	NULL	NULL	0	NULL	cisplatin	NULL		inhibit	NULL				pancreatic cancer	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevnutr_25_0_261_s_383	16011468	1-Methyl-propyl-2-imidazolozyl disulfide (PX-12), a TRX-1  inhibitor binding to the Cys73 residue, not only significantly potentiated the inhibitory  effect of cisplatin on pancreatic cancer ( 8) but also exhibited promising antitumor activities among a variety of tumor cell  lines both in vitro and in vivo ( 158).	bind
19382	4	6312	5	NULL	NULL	0	NULL	statement 1	NULL		potentiate	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevnutr_25_0_261_s_383	16011468	1-Methyl-propyl-2-imidazolozyl disulfide (PX-12), a TRX-1  inhibitor binding to the Cys73 residue, not only significantly potentiated the inhibitory  effect of cisplatin on pancreatic cancer ( 8) but also exhibited promising antitumor activities among a variety of tumor cell  lines both in vitro and in vivo ( 158).	bind
19383	5	6312	5	10	NULL	0	NULL	statement 1	NULL		exhibit	NULL				antitumor activities	NULL	promising			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_annurevnutr_25_0_261_s_383	16011468	1-Methyl-propyl-2-imidazolozyl disulfide (PX-12), a TRX-1  inhibitor binding to the Cys73 residue, not only significantly potentiated the inhibitory  effect of cisplatin on pancreatic cancer ( 8) but also exhibited promising antitumor activities among a variety of tumor cell  lines both in vitro and in vivo ( 158).	bind
19384	6	6312	5	10	NULL	0	NULL	statement 1	NULL		exhibit	NULL				antitumor activities	NULL	promising			NULL	in vivo	NULL	NULL	NULL	NULL	gw70_annurevnutr_25_0_261_s_383	16011468	1-Methyl-propyl-2-imidazolozyl disulfide (PX-12), a TRX-1  inhibitor binding to the Cys73 residue, not only significantly potentiated the inhibitory  effect of cisplatin on pancreatic cancer ( 8) but also exhibited promising antitumor activities among a variety of tumor cell  lines both in vitro and in vivo ( 158).	bind
54204	7	6312	5	10	NULL	0	NULL	PX-12			is an inhibitor of					TRX-1					NULL		0	NULL	NULL	NULL	gw70_annurevnutr_25_0_261_s_383	16011468	1-Methyl-propyl-2-imidazolozyl disulfide (PX-12), a TRX-1  inhibitor binding to the Cys73 residue, not only significantly potentiated the inhibitory  effect of cisplatin on pancreatic cancer ( 8) but also exhibited promising antitumor activities among a variety of tumor cell  lines both in vitro and in vivo ( 158).	bind
22053	1	6312	7	NULL	NULL	NULL	NULL	PX-12	Chemical		bind								Cys73 residue		NULL		NULL	NULL	NULL	NULL	gw70_annurevnutr_25_0_261_s_383	16011468	1-Methyl-propyl-2-imidazolozyl disulfide (PX-12), a TRX-1  inhibitor binding to the Cys73 residue, not only significantly potentiated the inhibitory  effect of cisplatin on pancreatic cancer ( 8) but also exhibited promising antitumor activities among a variety of tumor cell  lines both in vitro and in vivo ( 158).	bind
22054	2	6312	7	NULL	NULL	NULL	NULL	PX-12	Chemical		is					1-Methyl-propyl-2-imidazolozyl disulfide	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_annurevnutr_25_0_261_s_383	16011468	1-Methyl-propyl-2-imidazolozyl disulfide (PX-12), a TRX-1  inhibitor binding to the Cys73 residue, not only significantly potentiated the inhibitory  effect of cisplatin on pancreatic cancer ( 8) but also exhibited promising antitumor activities among a variety of tumor cell  lines both in vitro and in vivo ( 158).	bind
22055	3	6312	7	NULL	NULL	NULL	NULL	PX-12	Chemical		is an inhibitor of					TRX-1 	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevnutr_25_0_261_s_383	16011468	1-Methyl-propyl-2-imidazolozyl disulfide (PX-12), a TRX-1  inhibitor binding to the Cys73 residue, not only significantly potentiated the inhibitory  effect of cisplatin on pancreatic cancer ( 8) but also exhibited promising antitumor activities among a variety of tumor cell  lines both in vitro and in vivo ( 158).	bind
22056	4	6312	7	NULL	NULL	NULL	NULL	statement 1	Process		potentiate					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevnutr_25_0_261_s_383	16011468	1-Methyl-propyl-2-imidazolozyl disulfide (PX-12), a TRX-1  inhibitor binding to the Cys73 residue, not only significantly potentiated the inhibitory  effect of cisplatin on pancreatic cancer ( 8) but also exhibited promising antitumor activities among a variety of tumor cell  lines both in vitro and in vivo ( 158).	bind
22057	5	6312	7	NULL	NULL	NULL	NULL	PX-12	Chemical		activate					antitumor	Cell				NULL	invitro	NULL	NULL	NULL	NULL	gw70_annurevnutr_25_0_261_s_383	16011468	1-Methyl-propyl-2-imidazolozyl disulfide (PX-12), a TRX-1  inhibitor binding to the Cys73 residue, not only significantly potentiated the inhibitory  effect of cisplatin on pancreatic cancer ( 8) but also exhibited promising antitumor activities among a variety of tumor cell  lines both in vitro and in vivo ( 158).	bind
22058	6	6312	7	NULL	NULL	NULL	NULL	PX-12	Chemical		activate					antitumor	Cell				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_annurevnutr_25_0_261_s_383	16011468	1-Methyl-propyl-2-imidazolozyl disulfide (PX-12), a TRX-1  inhibitor binding to the Cys73 residue, not only significantly potentiated the inhibitory  effect of cisplatin on pancreatic cancer ( 8) but also exhibited promising antitumor activities among a variety of tumor cell  lines both in vitro and in vivo ( 158).	bind
54205	7	6312	7	NULL	NULL	NULL	NULL	cisplatin	Chemical		inhibits					pancreatic cancer	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw70_annurevnutr_25_0_261_s_383	16011468	1-Methyl-propyl-2-imidazolozyl disulfide (PX-12), a TRX-1  inhibitor binding to the Cys73 residue, not only significantly potentiated the inhibitory  effect of cisplatin on pancreatic cancer ( 8) but also exhibited promising antitumor activities among a variety of tumor cell  lines both in vitro and in vivo ( 158).	bind
19385	1	6318	5	NULL	NULL	0	NULL	cyclophilins	NULL		bind	NULL				cyclosporin A	NULL	immunosuppressant			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_2_968_s_14	16260779	1.8 [EC]): the cyclophilins, which bind the immunosuppressant cyclosporin A, the FK506-binding proteins, and the parvulins.	bind
54206	2	6318	5	10	NULL	0	NULL	cyclophilins			bind					FK506-binding proteins					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_2_968_s_14	16260779	1.8 [EC]): the cyclophilins, which bind the immunosuppressant cyclosporin A, the FK506-binding proteins, and the parvulins.	bind
54207	3	6318	5	10	NULL	0	NULL	cyclophilins			bind					parvulins					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_2_968_s_14	16260779	1.8 [EC]): the cyclophilins, which bind the immunosuppressant cyclosporin A, the FK506-binding proteins, and the parvulins.	bind
22060	1	6318	7	NULL	NULL	NULL	NULL	cyclophilins	GP		bind					cyclosporin A	Chemical	immunosuppressant			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_2_968_s_14	16260779	1.8 [EC]): the cyclophilins, which bind the immunosuppressant cyclosporin A, the FK506-binding proteins, and the parvulins.	bind
22061	2	6318	7	NULL	NULL	NULL	NULL	cyclophilins	GP		bind					FK506-binding proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_2_968_s_14	16260779	1.8 [EC]): the cyclophilins, which bind the immunosuppressant cyclosporin A, the FK506-binding proteins, and the parvulins.	bind
22063	3	6318	7	NULL	NULL	NULL	NULL	cyclophilins	GP		bind					parvulins	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_2_968_s_14	16260779	1.8 [EC]): the cyclophilins, which bind the immunosuppressant cyclosporin A, the FK506-binding proteins, and the parvulins.	bind
19386	1	6319	5	10	NULL	0	NULL	ColIb-P9 antisense Inc RNA	NULL		bind	NULL				RNA	NULL		5''-rUUGGCG-3'' motif in the loop sequence		NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_15_3145_s_285	11470871	10       Asano,K., Niimi,T., Yokoyama,S. and Mizobuchi,K. (1998) Structural basis for binding of the plasmid ColIb-P9 antisense Inc RNA to its target RNA with the 5''-rUUGGCG-3'' motif in the loop sequence.	bind
22071	1	6319	7	NULL	NULL	NULL	NULL	ColIb-P9 antisense Inc RNA	NucleicAcid		bind					RNA	NucleicAcid		5''-rUUGGCG-3'' motif in the loop sequence 		NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_15_3145_s_285	11470871	10       Asano,K., Niimi,T., Yokoyama,S. and Mizobuchi,K. (1998) Structural basis for binding of the plasmid ColIb-P9 antisense Inc RNA to its target RNA with the 5''-rUUGGCG-3'' motif in the loop sequence.	bind
19387	1	6320	5	NULL	NULL	0	NULL	GSK3beta	NULL		bind	NULL				APC-beta-catenin complex	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_7_1410_s_290	11266540	10       Rubinfeld,B., Albert,I., Porfiri,E., Fiol,C., Munemitsu,S. and Polakis,P. (1996) Binding of GSK3beta to the APC-beta-catenin complex and regulation of complex assembly.	bind
19388	2	6320	5	NULL	NULL	0	NULL	GSK3beta	NULL		regulates	NULL				complex assembly	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_7_1410_s_290	11266540	10       Rubinfeld,B., Albert,I., Porfiri,E., Fiol,C., Munemitsu,S. and Polakis,P. (1996) Binding of GSK3beta to the APC-beta-catenin complex and regulation of complex assembly.	bind
22072	1	6320	7	NULL	NULL	NULL	NULL	GSK3beta	GP		bind					APC-beta-catenin complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_7_1410_s_290	11266540	10       Rubinfeld,B., Albert,I., Porfiri,E., Fiol,C., Munemitsu,S. and Polakis,P. (1996) Binding of GSK3beta to the APC-beta-catenin complex and regulation of complex assembly.	bind
29341	2	6320	7	NULL	NULL	NULL	NULL	GSK3beta	GP		regulates					complex assembly	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_7_1410_s_290	11266540	10       Rubinfeld,B., Albert,I., Porfiri,E., Fiol,C., Munemitsu,S. and Polakis,P. (1996) Binding of GSK3beta to the APC-beta-catenin complex and regulation of complex assembly.	bind
19389	1	6321	5	NULL	NULL	0	NULL	GS1 strand-specific DNA binding complex	NULL		is enriched in	NULL				brain	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_21_4433_s_256	11691931	10       Taira,E., Finkenstadt,P.M. and Baraban,J.M. (1998) Identification of translin and trax as components of the GS1 strand-specific DNA binding complex enriched in brain.	bind
19390	2	6321	5	NULL	NULL	0	NULL	translin	NULL		is a component of	NULL				GS1 strand-specific DNA binding complex	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_21_4433_s_256	11691931	10       Taira,E., Finkenstadt,P.M. and Baraban,J.M. (1998) Identification of translin and trax as components of the GS1 strand-specific DNA binding complex enriched in brain.	bind
19391	3	6321	5	NULL	NULL	0	NULL	trax	NULL		is a component of	NULL				GS1 strand-specific DNA binding complex	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_21_4433_s_256	11691931	10       Taira,E., Finkenstadt,P.M. and Baraban,J.M. (1998) Identification of translin and trax as components of the GS1 strand-specific DNA binding complex enriched in brain.	bind
22443	1	6321	7	NULL	NULL	NULL	NULL	translin	GP		is a component of					GS1 strand-specific DNA binding complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_21_4433_s_256	11691931	10       Taira,E., Finkenstadt,P.M. and Baraban,J.M. (1998) Identification of translin and trax as components of the GS1 strand-specific DNA binding complex enriched in brain.	bind
22444	2	6321	7	NULL	NULL	NULL	NULL	trax	GP		is a component of					GS1 strand-specific DNA binding complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_21_4433_s_256	11691931	10       Taira,E., Finkenstadt,P.M. and Baraban,J.M. (1998) Identification of translin and trax as components of the GS1 strand-specific DNA binding complex enriched in brain.	bind
29342	3	6321	7	NULL	NULL	NULL	NULL	GS1 strand-specific DNA binding complex	GP		is enriched in					brain	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_21_4433_s_256	11691931	10       Taira,E., Finkenstadt,P.M. and Baraban,J.M. (1998) Identification of translin and trax as components of the GS1 strand-specific DNA binding complex enriched in brain.	bind
23060	1	6322	5	10	NULL	0	NULL	beta2GPI	NULL		target	NULL				APLAs	NULL				NULL	at the EC surface	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_303	10669657	10  23 25 31  At the EC surface, beta2GPI or beta2GPI-phospholipid complexes were thought to be the main targets of APLAs, and it has been shown that both MoAbs and polyclonal anti-beta2GPI antibodies can upregulate adhesion molecule expression and interleukin-6 secretion after EC binding 24 32  and induce adherence of monocytes to ECs. 10 25  However, the binding of APLAs to the EC surface has never been clearly demonstrated and remains speculative in view of scarce evidence of the loss in membrane asymmetry.	bind
23061	2	6322	5	10	NULL	0	NULL	beta2GPI-phospholipid complexes	NULL		target	NULL				APLAs	NULL				NULL	at the EC surface	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_303	10669657	10  23 25 31  At the EC surface, beta2GPI or beta2GPI-phospholipid complexes were thought to be the main targets of APLAs, and it has been shown that both MoAbs and polyclonal anti-beta2GPI antibodies can upregulate adhesion molecule expression and interleukin-6 secretion after EC binding 24 32  and induce adherence of monocytes to ECs. 10 25  However, the binding of APLAs to the EC surface has never been clearly demonstrated and remains speculative in view of scarce evidence of the loss in membrane asymmetry.	bind
23062	3	6322	5	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_303	10669657	10  23 25 31  At the EC surface, beta2GPI or beta2GPI-phospholipid complexes were thought to be the main targets of APLAs, and it has been shown that both MoAbs and polyclonal anti-beta2GPI antibodies can upregulate adhesion molecule expression and interleukin-6 secretion after EC binding 24 32  and induce adherence of monocytes to ECs. 10 25  However, the binding of APLAs to the EC surface has never been clearly demonstrated and remains speculative in view of scarce evidence of the loss in membrane asymmetry.	bind
23063	4	6322	5	NULL	NULL	0	NULL	MoAbs	NULL		up-regulates	NULL				adhesion molecule	NULL	expression of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_303	10669657	10  23 25 31  At the EC surface, beta2GPI or beta2GPI-phospholipid complexes were thought to be the main targets of APLAs, and it has been shown that both MoAbs and polyclonal anti-beta2GPI antibodies can upregulate adhesion molecule expression and interleukin-6 secretion after EC binding 24 32  and induce adherence of monocytes to ECs. 10 25  However, the binding of APLAs to the EC surface has never been clearly demonstrated and remains speculative in view of scarce evidence of the loss in membrane asymmetry.	bind
23064	5	6322	5	NULL	NULL	0	NULL	polyclonal anti-beta2GPI antibodies	NULL		up-regulates	NULL				adhesion molecule	NULL	expression of-			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_303	10669657	10  23 25 31  At the EC surface, beta2GPI or beta2GPI-phospholipid complexes were thought to be the main targets of APLAs, and it has been shown that both MoAbs and polyclonal anti-beta2GPI antibodies can upregulate adhesion molecule expression and interleukin-6 secretion after EC binding 24 32  and induce adherence of monocytes to ECs. 10 25  However, the binding of APLAs to the EC surface has never been clearly demonstrated and remains speculative in view of scarce evidence of the loss in membrane asymmetry.	bind
23065	6	6322	5	NULL	NULL	0	NULL	MoAbs	NULL		up-regulates	NULL				interleukin-6	NULL	secretion of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_303	10669657	10  23 25 31  At the EC surface, beta2GPI or beta2GPI-phospholipid complexes were thought to be the main targets of APLAs, and it has been shown that both MoAbs and polyclonal anti-beta2GPI antibodies can upregulate adhesion molecule expression and interleukin-6 secretion after EC binding 24 32  and induce adherence of monocytes to ECs. 10 25  However, the binding of APLAs to the EC surface has never been clearly demonstrated and remains speculative in view of scarce evidence of the loss in membrane asymmetry.	bind
23066	7	6322	5	NULL	NULL	0	NULL	polyclonal anti-beta2GPI antibodies	NULL		up-regulates	NULL				interleukin-6	NULL	secretion of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_303	10669657	10  23 25 31  At the EC surface, beta2GPI or beta2GPI-phospholipid complexes were thought to be the main targets of APLAs, and it has been shown that both MoAbs and polyclonal anti-beta2GPI antibodies can upregulate adhesion molecule expression and interleukin-6 secretion after EC binding 24 32  and induce adherence of monocytes to ECs. 10 25  However, the binding of APLAs to the EC surface has never been clearly demonstrated and remains speculative in view of scarce evidence of the loss in membrane asymmetry.	bind
23067	8	6322	5	NULL	NULL	0	NULL	statement 4	NULL		occurs after	NULL				EC	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_303	10669657	10  23 25 31  At the EC surface, beta2GPI or beta2GPI-phospholipid complexes were thought to be the main targets of APLAs, and it has been shown that both MoAbs and polyclonal anti-beta2GPI antibodies can upregulate adhesion molecule expression and interleukin-6 secretion after EC binding 24 32  and induce adherence of monocytes to ECs. 10 25  However, the binding of APLAs to the EC surface has never been clearly demonstrated and remains speculative in view of scarce evidence of the loss in membrane asymmetry.	bind
23068	9	6322	5	NULL	NULL	0	NULL	statement 5	NULL		occurs after	NULL				EC	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_303	10669657	10  23 25 31  At the EC surface, beta2GPI or beta2GPI-phospholipid complexes were thought to be the main targets of APLAs, and it has been shown that both MoAbs and polyclonal anti-beta2GPI antibodies can upregulate adhesion molecule expression and interleukin-6 secretion after EC binding 24 32  and induce adherence of monocytes to ECs. 10 25  However, the binding of APLAs to the EC surface has never been clearly demonstrated and remains speculative in view of scarce evidence of the loss in membrane asymmetry.	bind
23069	10	6322	5	NULL	NULL	0	NULL	statement 6	NULL		occurs after	NULL				EC	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_303	10669657	10  23 25 31  At the EC surface, beta2GPI or beta2GPI-phospholipid complexes were thought to be the main targets of APLAs, and it has been shown that both MoAbs and polyclonal anti-beta2GPI antibodies can upregulate adhesion molecule expression and interleukin-6 secretion after EC binding 24 32  and induce adherence of monocytes to ECs. 10 25  However, the binding of APLAs to the EC surface has never been clearly demonstrated and remains speculative in view of scarce evidence of the loss in membrane asymmetry.	bind
23070	11	6322	5	NULL	NULL	0	NULL	statement 7	NULL		occurs after	NULL				EC	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_303	10669657	10  23 25 31  At the EC surface, beta2GPI or beta2GPI-phospholipid complexes were thought to be the main targets of APLAs, and it has been shown that both MoAbs and polyclonal anti-beta2GPI antibodies can upregulate adhesion molecule expression and interleukin-6 secretion after EC binding 24 32  and induce adherence of monocytes to ECs. 10 25  However, the binding of APLAs to the EC surface has never been clearly demonstrated and remains speculative in view of scarce evidence of the loss in membrane asymmetry.	bind
23071	12	6322	5	NULL	NULL	0	NULL	monocytes	NULL		adhere to	NULL				ECs	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_303	10669657	10  23 25 31  At the EC surface, beta2GPI or beta2GPI-phospholipid complexes were thought to be the main targets of APLAs, and it has been shown that both MoAbs and polyclonal anti-beta2GPI antibodies can upregulate adhesion molecule expression and interleukin-6 secretion after EC binding 24 32  and induce adherence of monocytes to ECs. 10 25  However, the binding of APLAs to the EC surface has never been clearly demonstrated and remains speculative in view of scarce evidence of the loss in membrane asymmetry.	bind
23072	13	6322	5	NULL	NULL	0	NULL	MoAbs	NULL		induces	NULL				statement 12	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_303	10669657	10  23 25 31  At the EC surface, beta2GPI or beta2GPI-phospholipid complexes were thought to be the main targets of APLAs, and it has been shown that both MoAbs and polyclonal anti-beta2GPI antibodies can upregulate adhesion molecule expression and interleukin-6 secretion after EC binding 24 32  and induce adherence of monocytes to ECs. 10 25  However, the binding of APLAs to the EC surface has never been clearly demonstrated and remains speculative in view of scarce evidence of the loss in membrane asymmetry.	bind
23073	14	6322	5	NULL	NULL	0	NULL	polyclonal anti-beta2GPI antibodies	NULL		induces	NULL				statement 12	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_303	10669657	10  23 25 31  At the EC surface, beta2GPI or beta2GPI-phospholipid complexes were thought to be the main targets of APLAs, and it has been shown that both MoAbs and polyclonal anti-beta2GPI antibodies can upregulate adhesion molecule expression and interleukin-6 secretion after EC binding 24 32  and induce adherence of monocytes to ECs. 10 25  However, the binding of APLAs to the EC surface has never been clearly demonstrated and remains speculative in view of scarce evidence of the loss in membrane asymmetry.	bind
22445	1	6322	7	NULL	NULL	NULL	NULL	APLAs	GP		target					beta2GPI	GP				NULL	at the EC surface	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_303	10669657	10  23 25 31  At the EC surface, beta2GPI or beta2GPI-phospholipid complexes were thought to be the main targets of APLAs, and it has been shown that both MoAbs and polyclonal anti-beta2GPI antibodies can upregulate adhesion molecule expression and interleukin-6 secretion after EC binding 24 32  and induce adherence of monocytes to ECs. 10 25  However, the binding of APLAs to the EC surface has never been clearly demonstrated and remains speculative in view of scarce evidence of the loss in membrane asymmetry.	bind
22446	2	6322	7	NULL	NULL	NULL	NULL	APLAs	GP		target					beta2GPI-phospholipid complex	GP				NULL	at the EC surface	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_303	10669657	10  23 25 31  At the EC surface, beta2GPI or beta2GPI-phospholipid complexes were thought to be the main targets of APLAs, and it has been shown that both MoAbs and polyclonal anti-beta2GPI antibodies can upregulate adhesion molecule expression and interleukin-6 secretion after EC binding 24 32  and induce adherence of monocytes to ECs. 10 25  However, the binding of APLAs to the EC surface has never been clearly demonstrated and remains speculative in view of scarce evidence of the loss in membrane asymmetry.	bind
45648	3	6322	7	NULL	NULL	NULL	NULL	MoAbs	GP		upregulate					adhesion molecule	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_303	10669657	10  23 25 31  At the EC surface, beta2GPI or beta2GPI-phospholipid complexes were thought to be the main targets of APLAs, and it has been shown that both MoAbs and polyclonal anti-beta2GPI antibodies can upregulate adhesion molecule expression and interleukin-6 secretion after EC binding 24 32  and induce adherence of monocytes to ECs. 10 25  However, the binding of APLAs to the EC surface has never been clearly demonstrated and remains speculative in view of scarce evidence of the loss in membrane asymmetry.	bind
45649	4	6322	7	NULL	NULL	NULL	NULL	polyclonal anti-beta2GPI antibodies 	GP		upregulate					adhesion molecule	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_303	10669657	10  23 25 31  At the EC surface, beta2GPI or beta2GPI-phospholipid complexes were thought to be the main targets of APLAs, and it has been shown that both MoAbs and polyclonal anti-beta2GPI antibodies can upregulate adhesion molecule expression and interleukin-6 secretion after EC binding 24 32  and induce adherence of monocytes to ECs. 10 25  However, the binding of APLAs to the EC surface has never been clearly demonstrated and remains speculative in view of scarce evidence of the loss in membrane asymmetry.	bind
45650	5	6322	7	NULL	NULL	NULL	NULL	MoAbs	GP		upregulate					interleukin-6	GP	secretion of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_303	10669657	10  23 25 31  At the EC surface, beta2GPI or beta2GPI-phospholipid complexes were thought to be the main targets of APLAs, and it has been shown that both MoAbs and polyclonal anti-beta2GPI antibodies can upregulate adhesion molecule expression and interleukin-6 secretion after EC binding 24 32  and induce adherence of monocytes to ECs. 10 25  However, the binding of APLAs to the EC surface has never been clearly demonstrated and remains speculative in view of scarce evidence of the loss in membrane asymmetry.	bind
45651	6	6322	7	NULL	NULL	NULL	NULL	polyclonal anti-beta2GPI antibodies	GP		upregulate					interleukin-6	GP	secretion of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_303	10669657	10  23 25 31  At the EC surface, beta2GPI or beta2GPI-phospholipid complexes were thought to be the main targets of APLAs, and it has been shown that both MoAbs and polyclonal anti-beta2GPI antibodies can upregulate adhesion molecule expression and interleukin-6 secretion after EC binding 24 32  and induce adherence of monocytes to ECs. 10 25  However, the binding of APLAs to the EC surface has never been clearly demonstrated and remains speculative in view of scarce evidence of the loss in membrane asymmetry.	bind
45652	7	6322	7	NULL	NULL	NULL	NULL	statement 3	Process		occurs after					EC	CellComponent	binding of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_303	10669657	10  23 25 31  At the EC surface, beta2GPI or beta2GPI-phospholipid complexes were thought to be the main targets of APLAs, and it has been shown that both MoAbs and polyclonal anti-beta2GPI antibodies can upregulate adhesion molecule expression and interleukin-6 secretion after EC binding 24 32  and induce adherence of monocytes to ECs. 10 25  However, the binding of APLAs to the EC surface has never been clearly demonstrated and remains speculative in view of scarce evidence of the loss in membrane asymmetry.	bind
45653	8	6322	7	NULL	NULL	NULL	NULL	statement 4	Process		occurs after					EC	CellComponent	binding of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_303	10669657	10  23 25 31  At the EC surface, beta2GPI or beta2GPI-phospholipid complexes were thought to be the main targets of APLAs, and it has been shown that both MoAbs and polyclonal anti-beta2GPI antibodies can upregulate adhesion molecule expression and interleukin-6 secretion after EC binding 24 32  and induce adherence of monocytes to ECs. 10 25  However, the binding of APLAs to the EC surface has never been clearly demonstrated and remains speculative in view of scarce evidence of the loss in membrane asymmetry.	bind
45654	9	6322	7	NULL	NULL	NULL	NULL	statement 5	Process		occurs after					EC	CellComponent	binding of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_303	10669657	10  23 25 31  At the EC surface, beta2GPI or beta2GPI-phospholipid complexes were thought to be the main targets of APLAs, and it has been shown that both MoAbs and polyclonal anti-beta2GPI antibodies can upregulate adhesion molecule expression and interleukin-6 secretion after EC binding 24 32  and induce adherence of monocytes to ECs. 10 25  However, the binding of APLAs to the EC surface has never been clearly demonstrated and remains speculative in view of scarce evidence of the loss in membrane asymmetry.	bind
45655	10	6322	7	NULL	NULL	NULL	NULL	statement 6	Process		occurs after					EC	CellComponent	binding of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_303	10669657	10  23 25 31  At the EC surface, beta2GPI or beta2GPI-phospholipid complexes were thought to be the main targets of APLAs, and it has been shown that both MoAbs and polyclonal anti-beta2GPI antibodies can upregulate adhesion molecule expression and interleukin-6 secretion after EC binding 24 32  and induce adherence of monocytes to ECs. 10 25  However, the binding of APLAs to the EC surface has never been clearly demonstrated and remains speculative in view of scarce evidence of the loss in membrane asymmetry.	bind
45656	11	6322	7	NULL	NULL	NULL	NULL	monocytes	Cell		adhere to					ECs	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_303	10669657	10  23 25 31  At the EC surface, beta2GPI or beta2GPI-phospholipid complexes were thought to be the main targets of APLAs, and it has been shown that both MoAbs and polyclonal anti-beta2GPI antibodies can upregulate adhesion molecule expression and interleukin-6 secretion after EC binding 24 32  and induce adherence of monocytes to ECs. 10 25  However, the binding of APLAs to the EC surface has never been clearly demonstrated and remains speculative in view of scarce evidence of the loss in membrane asymmetry.	bind
45657	12	6322	7	NULL	NULL	NULL	NULL	MoAbs	GP		induce					statement 11	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_303	10669657	10  23 25 31  At the EC surface, beta2GPI or beta2GPI-phospholipid complexes were thought to be the main targets of APLAs, and it has been shown that both MoAbs and polyclonal anti-beta2GPI antibodies can upregulate adhesion molecule expression and interleukin-6 secretion after EC binding 24 32  and induce adherence of monocytes to ECs. 10 25  However, the binding of APLAs to the EC surface has never been clearly demonstrated and remains speculative in view of scarce evidence of the loss in membrane asymmetry.	bind
45658	13	6322	7	NULL	NULL	NULL	NULL	polyclonal anti-beta2GPI antibodies	GP		induce					statement 11	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_303	10669657	10  23 25 31  At the EC surface, beta2GPI or beta2GPI-phospholipid complexes were thought to be the main targets of APLAs, and it has been shown that both MoAbs and polyclonal anti-beta2GPI antibodies can upregulate adhesion molecule expression and interleukin-6 secretion after EC binding 24 32  and induce adherence of monocytes to ECs. 10 25  However, the binding of APLAs to the EC surface has never been clearly demonstrated and remains speculative in view of scarce evidence of the loss in membrane asymmetry.	bind
45659	14	6322	7	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_303	10669657	10  23 25 31  At the EC surface, beta2GPI or beta2GPI-phospholipid complexes were thought to be the main targets of APLAs, and it has been shown that both MoAbs and polyclonal anti-beta2GPI antibodies can upregulate adhesion molecule expression and interleukin-6 secretion after EC binding 24 32  and induce adherence of monocytes to ECs. 10 25  However, the binding of APLAs to the EC surface has never been clearly demonstrated and remains speculative in view of scarce evidence of the loss in membrane asymmetry.	bind
19392	1	6323	5	10	NULL	0	NULL	SLIGRL			is a type of					synthetic PAR-2 hexapeptide agonist					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_10_1054_s_35	10827135	10  Accordingly, the present study uses SLIGRL (a synthetic PAR-2 hexapeptide agonist, which activates PAR-2 but not PAR-1 10 ) to test the hypothesis that incremental responses to SFLLRN over thrombin are due to the copresence of PAR-1 and PAR-2.	bind
19393	2	6323	5	NULL	NULL	0	NULL	SLIGRL	NULL		activates	NULL				PAR-2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_86_10_1054_s_35	10827135	10  Accordingly, the present study uses SLIGRL (a synthetic PAR-2 hexapeptide agonist, which activates PAR-2 but not PAR-1 10 ) to test the hypothesis that incremental responses to SFLLRN over thrombin are due to the copresence of PAR-1 and PAR-2.	bind
19394	3	6323	5	NULL	NULL	0	NULL	SLIGRL	NULL		does not activate	NULL				PAR-1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_86_10_1054_s_35	10827135	10  Accordingly, the present study uses SLIGRL (a synthetic PAR-2 hexapeptide agonist, which activates PAR-2 but not PAR-1 10 ) to test the hypothesis that incremental responses to SFLLRN over thrombin are due to the copresence of PAR-1 and PAR-2.	bind
22454	1	6323	7	NULL	NULL	NULL	NULL	SLIGRL	Chemical		activates					PAR-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_10_1054_s_35	10827135	10  Accordingly, the present study uses SLIGRL (a synthetic PAR-2 hexapeptide agonist, which activates PAR-2 but not PAR-1 10 ) to test the hypothesis that incremental responses to SFLLRN over thrombin are due to the copresence of PAR-1 and PAR-2.	bind
22455	2	6323	7	NULL	NULL	NULL	NULL	SLIGRL	Chemical		does not activate					PAR-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_10_1054_s_35	10827135	10  Accordingly, the present study uses SLIGRL (a synthetic PAR-2 hexapeptide agonist, which activates PAR-2 but not PAR-1 10 ) to test the hypothesis that incremental responses to SFLLRN over thrombin are due to the copresence of PAR-1 and PAR-2.	bind
22458	3	6323	7	NULL	NULL	NULL	NULL	 SLIGRL	Chemical		is a type of					synthetic PAR-2 hexapeptide agonist	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_10_1054_s_35	10827135	10  Accordingly, the present study uses SLIGRL (a synthetic PAR-2 hexapeptide agonist, which activates PAR-2 but not PAR-1 10 ) to test the hypothesis that incremental responses to SFLLRN over thrombin are due to the copresence of PAR-1 and PAR-2.	bind
22978	1	6324	5	NULL	NULL	0	NULL	c-Fosc-Jun	NULL		bind	NULL					NULL			LRE	NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_2_365_s_158	9081693	10  Conservation of the 15-bp spacing between the proximal AP-1 site and the kappaB site in the human and murine TF promoters 53  suggested that this separation might optimize the functional interaction between c-Fosc-Jun and c-Relp65 bound to the LRE.	bind
22979	2	6324	5	NULL	NULL	0	NULL	c-Relp65	NULL		bind	NULL					NULL			LRE	NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_2_365_s_158	9081693	10  Conservation of the 15-bp spacing between the proximal AP-1 site and the kappaB site in the human and murine TF promoters 53  suggested that this separation might optimize the functional interaction between c-Fosc-Jun and c-Relp65 bound to the LRE.	bind
22980	3	6324	5	NULL	NULL	0	NULL	statement 1	NULL		interacts with	NULL	functionally			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_2_365_s_158	9081693	10  Conservation of the 15-bp spacing between the proximal AP-1 site and the kappaB site in the human and murine TF promoters 53  suggested that this separation might optimize the functional interaction between c-Fosc-Jun and c-Relp65 bound to the LRE.	bind
22985	4	6324	5	NULL	NULL	0	NULL	TF	NULL	human	is seperated from	NULL			AP-1 site in promoter	TF	NULL	human		kappaB site in promoter	NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_2_365_s_158	9081693	10  Conservation of the 15-bp spacing between the proximal AP-1 site and the kappaB site in the human and murine TF promoters 53  suggested that this separation might optimize the functional interaction between c-Fosc-Jun and c-Relp65 bound to the LRE.	bind
22986	5	6324	5	NULL	NULL	0	NULL	statement 4	NULL	conservation of	suggests	NULL				statement 3	NULL	optimization of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_2_365_s_158	9081693	10  Conservation of the 15-bp spacing between the proximal AP-1 site and the kappaB site in the human and murine TF promoters 53  suggested that this separation might optimize the functional interaction between c-Fosc-Jun and c-Relp65 bound to the LRE.	bind
22987	6	6324	5	NULL	NULL	0	NULL	TF	NULL	murine	is seperated from	NULL			AP-1 site in promoter	TF	NULL	murine		kappaB site in promoter	NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_2_365_s_158	9081693	10  Conservation of the 15-bp spacing between the proximal AP-1 site and the kappaB site in the human and murine TF promoters 53  suggested that this separation might optimize the functional interaction between c-Fosc-Jun and c-Relp65 bound to the LRE.	bind
22988	7	6324	5	NULL	NULL	0	NULL	statement 6	NULL	conservation of	suggests	NULL				statement 3	NULL	optimization of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_2_365_s_158	9081693	10  Conservation of the 15-bp spacing between the proximal AP-1 site and the kappaB site in the human and murine TF promoters 53  suggested that this separation might optimize the functional interaction between c-Fosc-Jun and c-Relp65 bound to the LRE.	bind
22460	1	6324	7	NULL	NULL	NULL	NULL	c-Relp65	GP		bind									LRE	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_2_365_s_158	9081693	10  Conservation of the 15-bp spacing between the proximal AP-1 site and the kappaB site in the human and murine TF promoters 53  suggested that this separation might optimize the functional interaction between c-Fosc-Jun and c-Relp65 bound to the LRE.	bind
22461	2	6324	7	NULL	NULL	NULL	NULL	c-Fosc-Jun	GP		bind									LRE	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_2_365_s_158	9081693	10  Conservation of the 15-bp spacing between the proximal AP-1 site and the kappaB site in the human and murine TF promoters 53  suggested that this separation might optimize the functional interaction between c-Fosc-Jun and c-Relp65 bound to the LRE.	bind
22462	4	6324	7	NULL	NULL	NULL	NULL	TF	GP	human proximal	is separated from				 AP-1 site in promoter	TF	GP	human		kappaB site in promoter	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_2_365_s_158	9081693	10  Conservation of the 15-bp spacing between the proximal AP-1 site and the kappaB site in the human and murine TF promoters 53  suggested that this separation might optimize the functional interaction between c-Fosc-Jun and c-Relp65 bound to the LRE.	bind
22463	5	6324	7	NULL	NULL	NULL	NULL	statement 4	Process	conservation of	suggests					statement 3	Process	optimization of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_2_365_s_158	9081693	10  Conservation of the 15-bp spacing between the proximal AP-1 site and the kappaB site in the human and murine TF promoters 53  suggested that this separation might optimize the functional interaction between c-Fosc-Jun and c-Relp65 bound to the LRE.	bind
22464	6	6324	7	NULL	NULL	NULL	NULL	TF	GP	murine proximal	is separated from				 AP-1 site in promoter	TF	GP	murine		kappaB site in promoter	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_2_365_s_158	9081693	10  Conservation of the 15-bp spacing between the proximal AP-1 site and the kappaB site in the human and murine TF promoters 53  suggested that this separation might optimize the functional interaction between c-Fosc-Jun and c-Relp65 bound to the LRE.	bind
22465	7	6324	7	NULL	NULL	NULL	NULL	statement 6	Process	conservation of	suggests					statement 3	Process	optimization of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_2_365_s_158	9081693	10  Conservation of the 15-bp spacing between the proximal AP-1 site and the kappaB site in the human and murine TF promoters 53  suggested that this separation might optimize the functional interaction between c-Fosc-Jun and c-Relp65 bound to the LRE.	bind
29343	3	6324	7	NULL	NULL	NULL	NULL	statement 1	Process		functionally interacts with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_2_365_s_158	9081693	10  Conservation of the 15-bp spacing between the proximal AP-1 site and the kappaB site in the human and murine TF promoters 53  suggested that this separation might optimize the functional interaction between c-Fosc-Jun and c-Relp65 bound to the LRE.	bind
19395	1	6325	5	NULL	NULL	0	NULL	tissue factor	NULL	exposed	bind	NULL				factor VIIa	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_27	7586275	10  Exposed tissue factor binds to factor VIIa, an essential step in the initiation of the coagulation pathway.	bind
19396	2	6325	5	10	NULL	0	NULL	statement 1	NULL		leads to	NULL				coagulation pathway	NULL	initiation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_27	7586275	10  Exposed tissue factor binds to factor VIIa, an essential step in the initiation of the coagulation pathway.	bind
22466	1	6325	7	NULL	NULL	NULL	NULL	tissue factor	GP	exposed	binds to					factor VIIa	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_27	7586275	10  Exposed tissue factor binds to factor VIIa, an essential step in the initiation of the coagulation pathway.	bind
22467	2	6325	7	NULL	NULL	NULL	NULL	statement 1	Process		leads to					coagulation pathway	Process	initiation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_27	7586275	10  Exposed tissue factor binds to factor VIIa, an essential step in the initiation of the coagulation pathway.	bind
19405	1	6327	5	NULL	NULL	0	NULL	Heparin	NULL		used as	NULL	clinically			anticoagulant	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2251_s_44	10479670	10  Heparin has wide clinical use as an anticoagulant in the initial treatment of acute venous thromboembolism and unstable angina, 26 27  its main action being the acceleration of antithrombin-mediated inactivation of thrombin, FXa, and FIXa and the binding of thrombin by heparin cofactor II. 28 29	bind
19406	2	6327	5	NULL	NULL	0	NULL	acute venous thromboembolism	NULL	initial treatment of	require	NULL				Heparin	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2251_s_44	10479670	10  Heparin has wide clinical use as an anticoagulant in the initial treatment of acute venous thromboembolism and unstable angina, 26 27  its main action being the acceleration of antithrombin-mediated inactivation of thrombin, FXa, and FIXa and the binding of thrombin by heparin cofactor II. 28 29	bind
19407	3	6327	5	NULL	NULL	0	NULL	unstable angina	NULL	treatment of	require	NULL				Heparin	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2251_s_44	10479670	10  Heparin has wide clinical use as an anticoagulant in the initial treatment of acute venous thromboembolism and unstable angina, 26 27  its main action being the acceleration of antithrombin-mediated inactivation of thrombin, FXa, and FIXa and the binding of thrombin by heparin cofactor II. 28 29	bind
19408	4	6327	5	NULL	NULL	0	NULL	antithrombin	NULL		mediate	NULL				thrombin	NULL	inactivation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2251_s_44	10479670	10  Heparin has wide clinical use as an anticoagulant in the initial treatment of acute venous thromboembolism and unstable angina, 26 27  its main action being the acceleration of antithrombin-mediated inactivation of thrombin, FXa, and FIXa and the binding of thrombin by heparin cofactor II. 28 29	bind
19409	5	6327	5	NULL	NULL	0	NULL	Heparin	NULL		accelerate	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2251_s_44	10479670	10  Heparin has wide clinical use as an anticoagulant in the initial treatment of acute venous thromboembolism and unstable angina, 26 27  its main action being the acceleration of antithrombin-mediated inactivation of thrombin, FXa, and FIXa and the binding of thrombin by heparin cofactor II. 28 29	bind
19410	6	6327	5	NULL	NULL	0	NULL	antithrombin	NULL		mediate	NULL				FXa	NULL	inactivation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2251_s_44	10479670	10  Heparin has wide clinical use as an anticoagulant in the initial treatment of acute venous thromboembolism and unstable angina, 26 27  its main action being the acceleration of antithrombin-mediated inactivation of thrombin, FXa, and FIXa and the binding of thrombin by heparin cofactor II. 28 29	bind
19411	7	6327	5	NULL	NULL	0	NULL	Heparin	NULL		accelerate	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2251_s_44	10479670	10  Heparin has wide clinical use as an anticoagulant in the initial treatment of acute venous thromboembolism and unstable angina, 26 27  its main action being the acceleration of antithrombin-mediated inactivation of thrombin, FXa, and FIXa and the binding of thrombin by heparin cofactor II. 28 29	bind
19412	8	6327	5	NULL	NULL	0	NULL	antithrombin	NULL		mediate	NULL				FIXa	NULL	inactivation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2251_s_44	10479670	10  Heparin has wide clinical use as an anticoagulant in the initial treatment of acute venous thromboembolism and unstable angina, 26 27  its main action being the acceleration of antithrombin-mediated inactivation of thrombin, FXa, and FIXa and the binding of thrombin by heparin cofactor II. 28 29	bind
19413	9	6327	5	NULL	NULL	0	NULL	Heparin	NULL		accelerate	NULL				statement 8	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2251_s_44	10479670	10  Heparin has wide clinical use as an anticoagulant in the initial treatment of acute venous thromboembolism and unstable angina, 26 27  its main action being the acceleration of antithrombin-mediated inactivation of thrombin, FXa, and FIXa and the binding of thrombin by heparin cofactor II. 28 29	bind
19414	10	6327	5	NULL	NULL	0	NULL	heparin cofactor II	NULL		bind	NULL				thrombin	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2251_s_44	10479670	10  Heparin has wide clinical use as an anticoagulant in the initial treatment of acute venous thromboembolism and unstable angina, 26 27  its main action being the acceleration of antithrombin-mediated inactivation of thrombin, FXa, and FIXa and the binding of thrombin by heparin cofactor II. 28 29	bind
19415	11	6327	5	NULL	NULL	0	NULL	Heparin	NULL		accelerate	NULL				statement 10	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2251_s_44	10479670	10  Heparin has wide clinical use as an anticoagulant in the initial treatment of acute venous thromboembolism and unstable angina, 26 27  its main action being the acceleration of antithrombin-mediated inactivation of thrombin, FXa, and FIXa and the binding of thrombin by heparin cofactor II. 28 29	bind
22469	1	6327	7	NULL	NULL	NULL	NULL	antithrombin	GP		mediates					thrombin	GP	inactivation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2251_s_44	10479670	10  Heparin has wide clinical use as an anticoagulant in the initial treatment of acute venous thromboembolism and unstable angina, 26 27  its main action being the acceleration of antithrombin-mediated inactivation of thrombin, FXa, and FIXa and the binding of thrombin by heparin cofactor II. 28 29	bind
22470	2	6327	7	NULL	NULL	NULL	NULL	antithrombin	GP		mediates					FXa	GP	inactivation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2251_s_44	10479670	10  Heparin has wide clinical use as an anticoagulant in the initial treatment of acute venous thromboembolism and unstable angina, 26 27  its main action being the acceleration of antithrombin-mediated inactivation of thrombin, FXa, and FIXa and the binding of thrombin by heparin cofactor II. 28 29	bind
22471	3	6327	7	NULL	NULL	NULL	NULL	antithrombin	GP		mediates					FIXa	GP	inactivation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2251_s_44	10479670	10  Heparin has wide clinical use as an anticoagulant in the initial treatment of acute venous thromboembolism and unstable angina, 26 27  its main action being the acceleration of antithrombin-mediated inactivation of thrombin, FXa, and FIXa and the binding of thrombin by heparin cofactor II. 28 29	bind
22472	4	6327	7	NULL	NULL	NULL	NULL	Heparin	GP		accelerates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2251_s_44	10479670	10  Heparin has wide clinical use as an anticoagulant in the initial treatment of acute venous thromboembolism and unstable angina, 26 27  its main action being the acceleration of antithrombin-mediated inactivation of thrombin, FXa, and FIXa and the binding of thrombin by heparin cofactor II. 28 29	bind
22473	5	6327	7	NULL	NULL	NULL	NULL	Heparin	GP		accelerates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2251_s_44	10479670	10  Heparin has wide clinical use as an anticoagulant in the initial treatment of acute venous thromboembolism and unstable angina, 26 27  its main action being the acceleration of antithrombin-mediated inactivation of thrombin, FXa, and FIXa and the binding of thrombin by heparin cofactor II. 28 29	bind
22474	6	6327	7	NULL	NULL	NULL	NULL	Heparin	GP		accelerates					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2251_s_44	10479670	10  Heparin has wide clinical use as an anticoagulant in the initial treatment of acute venous thromboembolism and unstable angina, 26 27  its main action being the acceleration of antithrombin-mediated inactivation of thrombin, FXa, and FIXa and the binding of thrombin by heparin cofactor II. 28 29	bind
22475	7	6327	7	NULL	NULL	NULL	NULL	heparin cofactor II	GP		bind					thrombin	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2251_s_44	10479670	10  Heparin has wide clinical use as an anticoagulant in the initial treatment of acute venous thromboembolism and unstable angina, 26 27  its main action being the acceleration of antithrombin-mediated inactivation of thrombin, FXa, and FIXa and the binding of thrombin by heparin cofactor II. 28 29	bind
29386	8	6327	7	NULL	NULL	NULL	NULL	Heparin	GP		use as an					anticoagulant	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2251_s_44	10479670	10  Heparin has wide clinical use as an anticoagulant in the initial treatment of acute venous thromboembolism and unstable angina, 26 27  its main action being the acceleration of antithrombin-mediated inactivation of thrombin, FXa, and FIXa and the binding of thrombin by heparin cofactor II. 28 29	bind
29387	9	6327	7	NULL	NULL	NULL	NULL	Heparin	GP		is used in the					acute venous thromboembolism	MedicalFinding	initial treatment of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2251_s_44	10479670	10  Heparin has wide clinical use as an anticoagulant in the initial treatment of acute venous thromboembolism and unstable angina, 26 27  its main action being the acceleration of antithrombin-mediated inactivation of thrombin, FXa, and FIXa and the binding of thrombin by heparin cofactor II. 28 29	bind
29388	10	6327	7	NULL	NULL	NULL	NULL	Heparin	GP		is used in the 					unstable angina	MedicalFinding	initial treatment of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2251_s_44	10479670	10  Heparin has wide clinical use as an anticoagulant in the initial treatment of acute venous thromboembolism and unstable angina, 26 27  its main action being the acceleration of antithrombin-mediated inactivation of thrombin, FXa, and FIXa and the binding of thrombin by heparin cofactor II. 28 29	bind
19397	1	6328	5	10	NULL	0	NULL	apo(a)	NULL		bind	NULL				core protein of decorin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_6_707_s_208	10747008	10  In addition, apo(a) from Lp(a) binds to the core protein of decorin.	bind
45613	2	6328	5	10	NULL	0	NULL	apo(a)	NULL		is from	NULL				Lp(a)	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_86_6_707_s_208	10747008	10  In addition, apo(a) from Lp(a) binds to the core protein of decorin.	bind
22476	1	6328	7	NULL	NULL	NULL	NULL	apo(a)	GP		binds to					core protein of decorin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_6_707_s_208	10747008	10  In addition, apo(a) from Lp(a) binds to the core protein of decorin.	bind
22477	2	6328	7	NULL	NULL	NULL	NULL	apo(a)	GP		is from					Lp(a)	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_6_707_s_208	10747008	10  In addition, apo(a) from Lp(a) binds to the core protein of decorin.	bind
19398	1	6330	5	NULL	NULL	0	NULL	111In-VLDL	NULL		bind	NULL				basophils	NULL	human			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_1_17_s_239	7538422	10  In this study, 111In-VLDL bound to human basophils and mast cells and binding of VLDL to the LDL receptor were demonstrable.	bind
19399	2	6330	5	NULL	NULL	0	NULL	111In-VLDL	NULL		bind	NULL				mast cells	NULL	human			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_1_17_s_239	7538422	10  In this study, 111In-VLDL bound to human basophils and mast cells and binding of VLDL to the LDL receptor were demonstrable.	bind
19400	3	6330	5	NULL	NULL	0	NULL	VLDL	NULL		bind	NULL				LDL receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_1_17_s_239	7538422	10  In this study, 111In-VLDL bound to human basophils and mast cells and binding of VLDL to the LDL receptor were demonstrable.	bind
22478	1	6330	7	NULL	NULL	NULL	NULL	111In-VLDL	Chemical		bind					basophils	Cell	human			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_1_17_s_239	7538422	10  In this study, 111In-VLDL bound to human basophils and mast cells and binding of VLDL to the LDL receptor were demonstrable.	bind
22479	2	6330	7	NULL	NULL	NULL	NULL	111In-VLDL	Chemical		bind					mast cells	Cell	human			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_1_17_s_239	7538422	10  In this study, 111In-VLDL bound to human basophils and mast cells and binding of VLDL to the LDL receptor were demonstrable.	bind
22480	3	6330	7	NULL	NULL	NULL	NULL	VLDL	Chemical		bind					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_1_17_s_239	7538422	10  In this study, 111In-VLDL bound to human basophils and mast cells and binding of VLDL to the LDL receptor were demonstrable.	bind
19401	1	6331	5	NULL	NULL	0	NULL		NULL	cleavage of	disrupts	NULL		70 amino acids from the C-terminus		apoA-I	NULL		HDL receptor - binding domain		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_1_210_s_197	10634820	10  Indeed, a limited proteolysis study showed that cleavage of 70 amino acids from the  C-terminus resulted in disruption of the HDL receptor - binding domain of apoA-I.	bind
22481	1	6331	7	NULL	NULL	NULL	NULL			cleavage of 	disrupts			70 amino acids  of C-terminus		apoA-I	GP		HDL receptor - binding domain		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_1_210_s_197	10634820	10  Indeed, a limited proteolysis study showed that cleavage of 70 amino acids from the  C-terminus resulted in disruption of the HDL receptor - binding domain of apoA-I.	bind
19402	1	6332	5	NULL	NULL	0	NULL	IP3	NULL		bind	NULL				IP3 receptor	NULL				NULL	on the membrane of SR	NULL	NULL	NULL	NULL	gw60_circulation_94_2_190_s_22	8674178	10  IP3 then binds to an IP3 receptor on the membrane of the SR to mobilize the stored calcium ions (Ca2+) from the SR into the cytosol.	bind
19403	2	6332	5	10	NULL	0	NULL	statement 1			mobilize					Ca2+		stored			NULL		NULL	NULL	NULL	NULL	gw60_circulation_94_2_190_s_22	8674178	10  IP3 then binds to an IP3 receptor on the membrane of the SR to mobilize the stored calcium ions (Ca2+) from the SR into the cytosol.	bind
19404	3	6332	5	NULL	NULL	0	NULL	Ca2+	NULL		is	NULL				calcium ions	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_94_2_190_s_22	8674178	10  IP3 then binds to an IP3 receptor on the membrane of the SR to mobilize the stored calcium ions (Ca2+) from the SR into the cytosol.	bind
28691	4	6332	5	NULL	NULL	0	NULL	Ca2+	NULL	from SR	moves to	NULL				cytosol	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_94_2_190_s_22	8674178	10  IP3 then binds to an IP3 receptor on the membrane of the SR to mobilize the stored calcium ions (Ca2+) from the SR into the cytosol.	bind
22482	1	6332	7	NULL	NULL	NULL	NULL	IP3	Chemical		binds to					IP3 receptor	GP				NULL	membrane of the SR	NULL	NULL	NULL	NULL	gw60_circulation_94_2_190_s_22	8674178	10  IP3 then binds to an IP3 receptor on the membrane of the SR to mobilize the stored calcium ions (Ca2+) from the SR into the cytosol.	bind
22483	2	6332	7	NULL	NULL	NULL	NULL	statement 1	Process		mobilize					Ca2+	Chemical	stored			NULL		NULL	NULL	NULL	NULL	gw60_circulation_94_2_190_s_22	8674178	10  IP3 then binds to an IP3 receptor on the membrane of the SR to mobilize the stored calcium ions (Ca2+) from the SR into the cytosol.	bind
22484	3	6332	7	NULL	NULL	NULL	NULL	Ca2+	Chemical	From SR	move to					cytosol	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_circulation_94_2_190_s_22	8674178	10  IP3 then binds to an IP3 receptor on the membrane of the SR to mobilize the stored calcium ions (Ca2+) from the SR into the cytosol.	bind
22485	4	6332	7	NULL	NULL	NULL	NULL	Ca2+	Chemical		is					calcium ions	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulation_94_2_190_s_22	8674178	10  IP3 then binds to an IP3 receptor on the membrane of the SR to mobilize the stored calcium ions (Ca2+) from the SR into the cytosol.	bind
19416	1	6334	5	NULL	NULL	0	NULL	GRB2	NULL		bind	NULL				Shc	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_79_6_1167_s_259	8943955	10  On the other hand, generally, GRB2 is known to bind Shc in response to insulin and subsequently activates the p21ras pathway, including MAP kinase and p90RSK, and association of GRB2 with IRS-1 is not a major pathway for activation of the p21ras pathway.	bind
19417	2	6334	5	NULL	NULL	0	NULL	statement 1	NULL		occurs in response to	NULL				insulin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_79_6_1167_s_259	8943955	10  On the other hand, generally, GRB2 is known to bind Shc in response to insulin and subsequently activates the p21ras pathway, including MAP kinase and p90RSK, and association of GRB2 with IRS-1 is not a major pathway for activation of the p21ras pathway.	bind
19418	3	6334	5	NULL	NULL	0	NULL	statement 1	NULL		activates	NULL	subsequently			p21ras pathway	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_79_6_1167_s_259	8943955	10  On the other hand, generally, GRB2 is known to bind Shc in response to insulin and subsequently activates the p21ras pathway, including MAP kinase and p90RSK, and association of GRB2 with IRS-1 is not a major pathway for activation of the p21ras pathway.	bind
19419	4	6334	5	NULL	NULL	0	NULL	statement 1	NULL		activates	NULL	subsequently			 MAP kinase	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_79_6_1167_s_259	8943955	10  On the other hand, generally, GRB2 is known to bind Shc in response to insulin and subsequently activates the p21ras pathway, including MAP kinase and p90RSK, and association of GRB2 with IRS-1 is not a major pathway for activation of the p21ras pathway.	bind
19420	5	6334	5	NULL	NULL	0	NULL	statement 1	NULL		activates	NULL	subsequently			p90RSK	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_79_6_1167_s_259	8943955	10  On the other hand, generally, GRB2 is known to bind Shc in response to insulin and subsequently activates the p21ras pathway, including MAP kinase and p90RSK, and association of GRB2 with IRS-1 is not a major pathway for activation of the p21ras pathway.	bind
19421	6	6334	5	NULL	NULL	0	NULL	GRB2	NULL		associates with	NULL				IRS-1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_79_6_1167_s_259	8943955	10  On the other hand, generally, GRB2 is known to bind Shc in response to insulin and subsequently activates the p21ras pathway, including MAP kinase and p90RSK, and association of GRB2 with IRS-1 is not a major pathway for activation of the p21ras pathway.	bind
19422	7	6334	5	NULL	NULL	0	NULL	statement 6	NULL		is not required for	NULL				p21ras pathway	NULL	activation of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_6_1167_s_259	8943955	10  On the other hand, generally, GRB2 is known to bind Shc in response to insulin and subsequently activates the p21ras pathway, including MAP kinase and p90RSK, and association of GRB2 with IRS-1 is not a major pathway for activation of the p21ras pathway.	bind
22486	1	6334	7	NULL	NULL	NULL	NULL	 GRB2	GP		bind					Shc	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_6_1167_s_259	8943955	10  On the other hand, generally, GRB2 is known to bind Shc in response to insulin and subsequently activates the p21ras pathway, including MAP kinase and p90RSK, and association of GRB2 with IRS-1 is not a major pathway for activation of the p21ras pathway.	bind
22487	2	6334	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs in response to					insulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_6_1167_s_259	8943955	10  On the other hand, generally, GRB2 is known to bind Shc in response to insulin and subsequently activates the p21ras pathway, including MAP kinase and p90RSK, and association of GRB2 with IRS-1 is not a major pathway for activation of the p21ras pathway.	bind
22488	3	6334	7	NULL	NULL	NULL	NULL	statement 1	Process		activates		subsequently			p21ras pathway	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_6_1167_s_259	8943955	10  On the other hand, generally, GRB2 is known to bind Shc in response to insulin and subsequently activates the p21ras pathway, including MAP kinase and p90RSK, and association of GRB2 with IRS-1 is not a major pathway for activation of the p21ras pathway.	bind
22489	4	6334	7	NULL	NULL	NULL	NULL	statement 1	Process		activates		subsequently			MAP kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_6_1167_s_259	8943955	10  On the other hand, generally, GRB2 is known to bind Shc in response to insulin and subsequently activates the p21ras pathway, including MAP kinase and p90RSK, and association of GRB2 with IRS-1 is not a major pathway for activation of the p21ras pathway.	bind
22490	5	6334	7	NULL	NULL	NULL	NULL	statement 1	Process		activates		subsequently			p90RSK	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_6_1167_s_259	8943955	10  On the other hand, generally, GRB2 is known to bind Shc in response to insulin and subsequently activates the p21ras pathway, including MAP kinase and p90RSK, and association of GRB2 with IRS-1 is not a major pathway for activation of the p21ras pathway.	bind
22491	6	6334	7	NULL	NULL	NULL	NULL	GRB2	GP		associate with					IRS-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_6_1167_s_259	8943955	10  On the other hand, generally, GRB2 is known to bind Shc in response to insulin and subsequently activates the p21ras pathway, including MAP kinase and p90RSK, and association of GRB2 with IRS-1 is not a major pathway for activation of the p21ras pathway.	bind
22492	7	6334	7	NULL	NULL	NULL	NULL	statement 6	Process		 is not required for					p21ras pathway	Process	 activation of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_6_1167_s_259	8943955	10  On the other hand, generally, GRB2 is known to bind Shc in response to insulin and subsequently activates the p21ras pathway, including MAP kinase and p90RSK, and association of GRB2 with IRS-1 is not a major pathway for activation of the p21ras pathway.	bind
19423	1	6335	5	NULL	NULL	0	NULL	FXa	NULL		bind	NULL				TF	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2251_s_30	10479670	10  TFPI uses the tandem Kunitz-type domains in its structure to form a quaternary complex with FXa bound to TF .	bind
19424	2	6335	5	NULL	NULL	0	NULL	TFPI	NULL		bind	NULL		tandem Kunitz-type domains		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2251_s_30	10479670	10  TFPI uses the tandem Kunitz-type domains in its structure to form a quaternary complex with FXa bound to TF .	bind
28692	3	6335	5	NULL	NULL	0	NULL	statement 2	NULL		forms	NULL				quaternary complex	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2251_s_30	10479670	10  TFPI uses the tandem Kunitz-type domains in its structure to form a quaternary complex with FXa bound to TF .	bind
22493	1	6335	7	NULL	NULL	NULL	NULL	FXa	GP		bind					TF	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2251_s_30	10479670	10  TFPI uses the tandem Kunitz-type domains in its structure to form a quaternary complex with FXa bound to TF .	bind
22494	3	6335	7	NULL	NULL	NULL	NULL	statement 2	Process		forms					quaternary complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2251_s_30	10479670	10  TFPI uses the tandem Kunitz-type domains in its structure to form a quaternary complex with FXa bound to TF .	bind
22495	2	6335	7	NULL	NULL	NULL	NULL	TFPI	GP		bind			tandem Kunitz-type domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2251_s_30	10479670	10  TFPI uses the tandem Kunitz-type domains in its structure to form a quaternary complex with FXa bound to TF .	bind
19425	1	6336	5	NULL	NULL	0	NULL	follistatin	NULL		regulates	NULL				activin	NULL	activity of			NULL		0	NULL	NULL	NULL	gw60_circulationres_85_10_931_s_19	10559140	10  The activity of activin is regulated by follistatin, a 34-kDa glycoprotein, which binds activin with high affinity in equimolar complexes that are unable to bind and activate the activin receptors.	bind
19426	2	6336	5	NULL	NULL	0	NULL	follistatin	NULL		bind	NULL	high affinity			activin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_10_931_s_19	10559140	10  The activity of activin is regulated by follistatin, a 34-kDa glycoprotein, which binds activin with high affinity in equimolar complexes that are unable to bind and activate the activin receptors.	bind
19427	3	6336	5	NULL	NULL	0	NULL	statement 2	NULL		does not bind	NULL				activin receptors	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_10_931_s_19	10559140	10  The activity of activin is regulated by follistatin, a 34-kDa glycoprotein, which binds activin with high affinity in equimolar complexes that are unable to bind and activate the activin receptors.	bind
19428	4	6336	5	NULL	NULL	0	NULL	statement 2	NULL		does not activate	NULL				activin receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_85_10_931_s_19	10559140	10  The activity of activin is regulated by follistatin, a 34-kDa glycoprotein, which binds activin with high affinity in equimolar complexes that are unable to bind and activate the activin receptors.	bind
28693	5	6336	5	NULL	NULL	0	NULL	follistatin	NULL		is a type of	NULL				34-kDa glycoprotein	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_85_10_931_s_19	10559140	10  The activity of activin is regulated by follistatin, a 34-kDa glycoprotein, which binds activin with high affinity in equimolar complexes that are unable to bind and activate the activin receptors.	bind
22496	1	6336	7	NULL	NULL	NULL	NULL	follistatin	GP		binds		high affinity			activin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_10_931_s_19	10559140	10  The activity of activin is regulated by follistatin, a 34-kDa glycoprotein, which binds activin with high affinity in equimolar complexes that are unable to bind and activate the activin receptors.	bind
22497	2	6336	7	NULL	NULL	NULL	NULL	follistatin	GP		regulates					activin	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_10_931_s_19	10559140	10  The activity of activin is regulated by follistatin, a 34-kDa glycoprotein, which binds activin with high affinity in equimolar complexes that are unable to bind and activate the activin receptors.	bind
22498	3	6336	7	NULL	NULL	NULL	NULL	follistatin	GP		is a type of					34-kDa glycoprotein	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_10_931_s_19	10559140	10  The activity of activin is regulated by follistatin, a 34-kDa glycoprotein, which binds activin with high affinity in equimolar complexes that are unable to bind and activate the activin receptors.	bind
22499	4	6336	7	NULL	NULL	NULL	NULL	statement 1	Process		does not bind					activin receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_10_931_s_19	10559140	10  The activity of activin is regulated by follistatin, a 34-kDa glycoprotein, which binds activin with high affinity in equimolar complexes that are unable to bind and activate the activin receptors.	bind
22500	5	6336	7	NULL	NULL	NULL	NULL	statement 1	Process		does not activate					activin receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_10_931_s_19	10559140	10  The activity of activin is regulated by follistatin, a 34-kDa glycoprotein, which binds activin with high affinity in equimolar complexes that are unable to bind and activate the activin receptors.	bind
19429	1	6337	5	10	NULL	0	NULL	hirudin			bind					fibrinogen			recognition exosite		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_10_987_s_36	11375267	10  The exogenous leech - derived inhibitor hirudin also binds to the fibrinogen-recognition exosite and the active site to inhibit thrombin function 11  and is used clinically as a potent antithrombin.	bind
19430	2	6337	5	10	NULL	0	NULL	hirudin			bind					fibrinogen			active site		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_10_987_s_36	11375267	10  The exogenous leech - derived inhibitor hirudin also binds to the fibrinogen-recognition exosite and the active site to inhibit thrombin function 11  and is used clinically as a potent antithrombin.	bind
19431	3	6337	5	NULL	NULL	0	NULL	statement 1	NULL		inhibit	NULL				thrombin	NULL	function of			NULL		0	NULL	NULL	NULL	gw60_circulationres_88_10_987_s_36	11375267	10  The exogenous leech - derived inhibitor hirudin also binds to the fibrinogen-recognition exosite and the active site to inhibit thrombin function 11  and is used clinically as a potent antithrombin.	bind
19432	4	6337	5	NULL	NULL	0	NULL	statement 2	NULL		inhibit	NULL				thrombin	NULL	function of			NULL		0	NULL	NULL	NULL	gw60_circulationres_88_10_987_s_36	11375267	10  The exogenous leech - derived inhibitor hirudin also binds to the fibrinogen-recognition exosite and the active site to inhibit thrombin function 11  and is used clinically as a potent antithrombin.	bind
19433	5	6337	5	10	NULL	0	NULL	hirudin			is used as		clinically			antithrombin		potent			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_10_987_s_36	11375267	10  The exogenous leech - derived inhibitor hirudin also binds to the fibrinogen-recognition exosite and the active site to inhibit thrombin function 11  and is used clinically as a potent antithrombin.	bind
54208	5	6337	5	10	NULL	0	NULL	hirudin			is a type of					exogenous leech - derived inhibitor					NULL		0	NULL	NULL	NULL	gw60_circulationres_88_10_987_s_36	11375267	10  The exogenous leech - derived inhibitor hirudin also binds to the fibrinogen-recognition exosite and the active site to inhibit thrombin function 11  and is used clinically as a potent antithrombin.	bind
22501	1	6337	7	NULL	NULL	NULL	NULL	hirudin	GP		binds to					fibrinogen	GP		recognition exosite		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_10_987_s_36	11375267	10  The exogenous leech - derived inhibitor hirudin also binds to the fibrinogen-recognition exosite and the active site to inhibit thrombin function 11  and is used clinically as a potent antithrombin.	bind
22502	2	6337	7	NULL	NULL	NULL	NULL	hirudin	GP		binds to					fibrinogen	GP		active site		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_10_987_s_36	11375267	10  The exogenous leech - derived inhibitor hirudin also binds to the fibrinogen-recognition exosite and the active site to inhibit thrombin function 11  and is used clinically as a potent antithrombin.	bind
22503	3	6337	7	NULL	NULL	NULL	NULL	statement 1	Process		inhibit					thrombin	GP	function of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_10_987_s_36	11375267	10  The exogenous leech - derived inhibitor hirudin also binds to the fibrinogen-recognition exosite and the active site to inhibit thrombin function 11  and is used clinically as a potent antithrombin.	bind
22504	4	6337	7	NULL	NULL	NULL	NULL	statement 2	Process		inhibit					thrombin	GP	function of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_10_987_s_36	11375267	10  The exogenous leech - derived inhibitor hirudin also binds to the fibrinogen-recognition exosite and the active site to inhibit thrombin function 11  and is used clinically as a potent antithrombin.	bind
22505	5	6337	7	NULL	NULL	NULL	NULL	hirudin	GP		is used as		clinically			antithrombin	GP	potent			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_10_987_s_36	11375267	10  The exogenous leech - derived inhibitor hirudin also binds to the fibrinogen-recognition exosite and the active site to inhibit thrombin function 11  and is used clinically as a potent antithrombin.	bind
54209	6	6337	7	NULL	NULL	NULL	NULL	hirudin	GP		is a type of					exogenous leech - derived inhibitor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_10_987_s_36	11375267	10  The exogenous leech - derived inhibitor hirudin also binds to the fibrinogen-recognition exosite and the active site to inhibit thrombin function 11  and is used clinically as a potent antithrombin.	bind
19434	1	6338	5	NULL	NULL	0	NULL		NULL		bind	NULL		tryptophan-rich motif within the type 1 repeats		heparin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_100_13_1423_s_24	10500044	10  The peptides used in these assays included a tryptophan-rich motif within the type 1 repeats that binds to heparin.	bind
22506	1	6338	7	NULL	NULL	NULL	NULL				bind			tryptophan-rich motif within type 1 repeat		heparin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_13_1423_s_24	10500044	10  The peptides used in these assays included a tryptophan-rich motif within the type 1 repeats that binds to heparin.	bind
19435	1	6339	5	NULL	NULL	0	NULL	heparin	NULL		bind	NULL					NULL		I domain		NULL		0	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_158	10510057	10  Therefore, our data could be explained by binding of heparin to the I domain which may then cause steric hindrance of the binding of factor X to spatially distinct binding sites within Mac-1.	bind
19436	2	6339	5	NULL	NULL	0	NULL	factor X	NULL		bind	NULL				Mac-1	NULL	spatially distinct binding sites			NULL		0	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_158	10510057	10  Therefore, our data could be explained by binding of heparin to the I domain which may then cause steric hindrance of the binding of factor X to spatially distinct binding sites within Mac-1.	bind
19437	3	6339	5	NULL	NULL	0	NULL	statement 1	NULL		cause	NULL	may			statement 2	NULL	steric hindrance of			NULL		0	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_158	10510057	10  Therefore, our data could be explained by binding of heparin to the I domain which may then cause steric hindrance of the binding of factor X to spatially distinct binding sites within Mac-1.	bind
22507	1	6339	7	NULL	NULL	NULL	NULL	 heparin	GP		bind								I domain		NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_158	10510057	10  Therefore, our data could be explained by binding of heparin to the I domain which may then cause steric hindrance of the binding of factor X to spatially distinct binding sites within Mac-1.	bind
22508	2	6339	7	NULL	NULL	NULL	NULL	factor X	GP		bind					Mac-1	GP		spatially distinct binding site within		NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_158	10510057	10  Therefore, our data could be explained by binding of heparin to the I domain which may then cause steric hindrance of the binding of factor X to spatially distinct binding sites within Mac-1.	bind
22509	3	6339	7	NULL	NULL	NULL	NULL	statement 1	Process		cause		may			statement 2	Process	steric hindrance of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_158	10510057	10  Therefore, our data could be explained by binding of heparin to the I domain which may then cause steric hindrance of the binding of factor X to spatially distinct binding sites within Mac-1.	bind
19438	1	6340	5	10	NULL	0	NULL	PAI-1			bind					vitronectin					NULL	vascular smooth muscle cells	NULL	NULL	NULL	NULL	gw60_circulation_103_25_3105_s_25	11425776	10  This effect appears to be mediated by inhibition of plasmin formation and possibly by PAI-1 binding to vitronectin, thereby preventing its interaction with vitronectin receptors present on vascular smooth muscle cells.	bind
19439	2	6340	5	NULL	NULL	0	NULL	PAI-1	NULL		interacts with	NULL				vitronectin receptors	NULL				NULL	on vascular smooth muscle cells	NULL	NULL	NULL	NULL	gw60_circulation_103_25_3105_s_25	11425776	10  This effect appears to be mediated by inhibition of plasmin formation and possibly by PAI-1 binding to vitronectin, thereby preventing its interaction with vitronectin receptors present on vascular smooth muscle cells.	bind
28694	3	6340	5	10	NULL	0	NULL	statement 1			prevents					statement 2					NULL	vascular smooth muscle cells	NULL	NULL	NULL	NULL	gw60_circulation_103_25_3105_s_25	11425776	10  This effect appears to be mediated by inhibition of plasmin formation and possibly by PAI-1 binding to vitronectin, thereby preventing its interaction with vitronectin receptors present on vascular smooth muscle cells.	bind
22510	1	6340	7	NULL	NULL	NULL	NULL	 PAI-1	GP		bind					vitronectin	GP				NULL	vascular smooth muscle cells	NULL	NULL	NULL	NULL	gw60_circulation_103_25_3105_s_25	11425776	10  This effect appears to be mediated by inhibition of plasmin formation and possibly by PAI-1 binding to vitronectin, thereby preventing its interaction with vitronectin receptors present on vascular smooth muscle cells.	bind
22511	2	6340	7	NULL	NULL	NULL	NULL	PAI-1	GP		binds					vitronectin receptors	GP				NULL	vascular smooth muscle cells	NULL	NULL	NULL	NULL	gw60_circulation_103_25_3105_s_25	11425776	10  This effect appears to be mediated by inhibition of plasmin formation and possibly by PAI-1 binding to vitronectin, thereby preventing its interaction with vitronectin receptors present on vascular smooth muscle cells.	bind
22512	3	6340	7	NULL	NULL	NULL	NULL	statement 1	Process		prevents					statement 2	Process				NULL	vascular smooth muscle cells	NULL	NULL	NULL	NULL	gw60_circulation_103_25_3105_s_25	11425776	10  This effect appears to be mediated by inhibition of plasmin formation and possibly by PAI-1 binding to vitronectin, thereby preventing its interaction with vitronectin receptors present on vascular smooth muscle cells.	bind
19440	1	6342	5	NULL	NULL	0	NULL	osteonectin	NULL		bind	NULL				plasminogen	NULL				NULL	 in ECs	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_8_1852_s_29	10446063	10 11 12  Recently, it has been shown that osteonectin binds to plasminogen, 13 increases its activation and binding to collagen, 13  and induces the expression of type 1 plasminogen activator inhibitor in endothelial cells (ECs).	bind
19441	2	6342	5	NULL	NULL	0	NULL	osteonectin	NULL		increases	NULL				plasminogen	NULL	activation of			NULL	in ECs	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_8_1852_s_29	10446063	10 11 12  Recently, it has been shown that osteonectin binds to plasminogen, 13 increases its activation and binding to collagen, 13  and induces the expression of type 1 plasminogen activator inhibitor in endothelial cells (ECs).	bind
19442	3	6342	5	NULL	NULL	0	NULL	plasminogen	NULL		bind	NULL				collagen	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_8_1852_s_29	10446063	10 11 12  Recently, it has been shown that osteonectin binds to plasminogen, 13 increases its activation and binding to collagen, 13  and induces the expression of type 1 plasminogen activator inhibitor in endothelial cells (ECs).	bind
19443	4	6342	5	NULL	NULL	0	NULL	osteonectin	NULL		increases	NULL				statement 3	NULL				NULL	in ECs	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_8_1852_s_29	10446063	10 11 12  Recently, it has been shown that osteonectin binds to plasminogen, 13 increases its activation and binding to collagen, 13  and induces the expression of type 1 plasminogen activator inhibitor in endothelial cells (ECs).	bind
19444	5	6342	5	NULL	NULL	0	NULL	osteonectin	NULL		induces	NULL				type 1 plasminogen activator inhibitor	NULL	expression of			NULL	in ECs	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_8_1852_s_29	10446063	10 11 12  Recently, it has been shown that osteonectin binds to plasminogen, 13 increases its activation and binding to collagen, 13  and induces the expression of type 1 plasminogen activator inhibitor in endothelial cells (ECs).	bind
28695	6	6342	5	NULL	NULL	0	NULL	ECs	NULL		is	NULL				endothelial cells	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_8_1852_s_29	10446063	10 11 12  Recently, it has been shown that osteonectin binds to plasminogen, 13 increases its activation and binding to collagen, 13  and induces the expression of type 1 plasminogen activator inhibitor in endothelial cells (ECs).	bind
22513	1	6342	7	NULL	NULL	NULL	NULL	osteonectin	GP		binds to					plasminogen	GP				NULL	in ECs	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_8_1852_s_29	10446063	10 11 12  Recently, it has been shown that osteonectin binds to plasminogen, 13 increases its activation and binding to collagen, 13  and induces the expression of type 1 plasminogen activator inhibitor in endothelial cells (ECs).	bind
22514	2	6342	7	NULL	NULL	NULL	NULL	statement 1	Process		increases					plasminogen	GP	activation of			NULL	in ECs	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_8_1852_s_29	10446063	10 11 12  Recently, it has been shown that osteonectin binds to plasminogen, 13 increases its activation and binding to collagen, 13  and induces the expression of type 1 plasminogen activator inhibitor in endothelial cells (ECs).	bind
22515	3	6342	7	NULL	NULL	NULL	NULL	plasminogen	GP		binds to					collagen	GP				NULL	in ECs	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_8_1852_s_29	10446063	10 11 12  Recently, it has been shown that osteonectin binds to plasminogen, 13 increases its activation and binding to collagen, 13  and induces the expression of type 1 plasminogen activator inhibitor in endothelial cells (ECs).	bind
22516	4	6342	7	NULL	NULL	NULL	NULL	statement 1	Process		increases					statement 3	Process				NULL	in ECs	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_8_1852_s_29	10446063	10 11 12  Recently, it has been shown that osteonectin binds to plasminogen, 13 increases its activation and binding to collagen, 13  and induces the expression of type 1 plasminogen activator inhibitor in endothelial cells (ECs).	bind
22517	5	6342	7	NULL	NULL	NULL	NULL	osteonectin	GP		induces					type 1 plasminogen activator inhibitor	GP	expression of			NULL	in ECs	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_8_1852_s_29	10446063	10 11 12  Recently, it has been shown that osteonectin binds to plasminogen, 13 increases its activation and binding to collagen, 13  and induces the expression of type 1 plasminogen activator inhibitor in endothelial cells (ECs).	bind
22518	6	6342	7	NULL	NULL	NULL	NULL	ECs	Cell		is					Endothelial cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_8_1852_s_29	10446063	10 11 12  Recently, it has been shown that osteonectin binds to plasminogen, 13 increases its activation and binding to collagen, 13  and induces the expression of type 1 plasminogen activator inhibitor in endothelial cells (ECs).	bind
22989	1	6344	5	NULL	NULL	0	NULL	GR	NULL	endogenous	bind	NULL					NULL			glucocorticoid-response element	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_33_30031_s_155	12039962	10 7M dexamethasone was added to activate the gene by the endogenous GR binding to the glucocorticoid-response element located from  333 to  319 of the promoter Ib sequence.	bind
22990	2	6344	5	10	NULL	0	NULL				is located from				glucocorticoid-response element					333 to 319 of promoter Ib sequence	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_33_30031_s_155	12039962	10 7M dexamethasone was added to activate the gene by the endogenous GR binding to the glucocorticoid-response element located from  333 to  319 of the promoter Ib sequence.	bind
22544	1	6344	7	NULL	NULL	NULL	NULL	GR	GP	endogenous	bind									glucocorticoid-response element	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_33_30031_s_155	12039962	10 7M dexamethasone was added to activate the gene by the endogenous GR binding to the glucocorticoid-response element located from  333 to  319 of the promoter Ib sequence.	bind
22545	2	6344	7	NULL	NULL	0	NULL		NULL		located	NULL			glucocorticoid-response element		NULL			 from 333 to 319 of the promoter Ib sequence	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_33_30031_s_155	12039962	10 7M dexamethasone was added to activate the gene by the endogenous GR binding to the glucocorticoid-response element located from  333 to  319 of the promoter Ib sequence.	bind
22546	3	6344	7	NULL	NULL	NULL	NULL	dexamethasone	Chemical		activate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_33_30031_s_155	12039962	10 7M dexamethasone was added to activate the gene by the endogenous GR binding to the glucocorticoid-response element located from  333 to  319 of the promoter Ib sequence.	bind
19445	1	6345	5	NULL	NULL	0	NULL	AcrB	NULL		bind	NULL	directly			TolC	NULL				NULL		0	NULL	NULL	NULL	gw60_jantimicrobchemoth_52_2_176_s_84	12837741	10 According to the three-dimensional structure, AcrB directly binds to TolC.	bind
22549	1	6345	7	NULL	NULL	NULL	NULL	AcrB	GP		binds to		directly			TolC	GP				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_52_2_176_s_84	12837741	10 According to the three-dimensional structure, AcrB directly binds to TolC.	bind
19477	1	6346	5	NULL	NULL	0	NULL	beta3 peptide	NULL	diphosphorylated	bind	NULL				myosin	NULL	purified			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_22_13878_s_172	9593734	10 mM phenylphosphate inhibited completely the binding of the diphosphorylated beta3 peptide to purified myosin in renatured blots (Fig.  4 C), indicating that the beta3-myosin interaction was phosphotyrosine-dependent under these binding conditions.	bind
19478	2	6346	5	NULL	NULL	0	NULL	phenylphosphate	NULL		inhibit	NULL	completely			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_22_13878_s_172	9593734	10 mM phenylphosphate inhibited completely the binding of the diphosphorylated beta3 peptide to purified myosin in renatured blots (Fig.  4 C), indicating that the beta3-myosin interaction was phosphotyrosine-dependent under these binding conditions.	bind
19479	3	6346	5	10	NULL	0	NULL	statement 1			is dependent on								phosphotyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_22_13878_s_172	9593734	10 mM phenylphosphate inhibited completely the binding of the diphosphorylated beta3 peptide to purified myosin in renatured blots (Fig.  4 C), indicating that the beta3-myosin interaction was phosphotyrosine-dependent under these binding conditions.	bind
19480	4	6346	5	NULL	NULL	0	NULL	statement 2	NULL		indicates	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_22_13878_s_172	9593734	10 mM phenylphosphate inhibited completely the binding of the diphosphorylated beta3 peptide to purified myosin in renatured blots (Fig.  4 C), indicating that the beta3-myosin interaction was phosphotyrosine-dependent under these binding conditions.	bind
22550	1	6346	7	NULL	NULL	NULL	NULL	  beta3 peptide	GP	diphosphorylated	binds					myosin	GP	purified			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_22_13878_s_172	9593734	10 mM phenylphosphate inhibited completely the binding of the diphosphorylated beta3 peptide to purified myosin in renatured blots (Fig.  4 C), indicating that the beta3-myosin interaction was phosphotyrosine-dependent under these binding conditions.	bind
22551	2	6346	7	NULL	NULL	NULL	NULL	statement 1	Process		depends on								phosphotyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_22_13878_s_172	9593734	10 mM phenylphosphate inhibited completely the binding of the diphosphorylated beta3 peptide to purified myosin in renatured blots (Fig.  4 C), indicating that the beta3-myosin interaction was phosphotyrosine-dependent under these binding conditions.	bind
22552	3	6346	7	NULL	NULL	NULL	NULL	phenylphosphate	Chemical		inhibits		completely			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_22_13878_s_172	9593734	10 mM phenylphosphate inhibited completely the binding of the diphosphorylated beta3 peptide to purified myosin in renatured blots (Fig.  4 C), indicating that the beta3-myosin interaction was phosphotyrosine-dependent under these binding conditions.	bind
29389	4	6346	7	NULL	NULL	NULL	NULL	statement 3	Process		indicates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_22_13878_s_172	9593734	10 mM phenylphosphate inhibited completely the binding of the diphosphorylated beta3 peptide to purified myosin in renatured blots (Fig.  4 C), indicating that the beta3-myosin interaction was phosphotyrosine-dependent under these binding conditions.	bind
19481	1	6351	5	NULL	NULL	0	NULL	Tel-2b	NULL		bind	NULL				E74 probe	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_12_9421_s_308	11108721	10 ng of wild-type competitor completely abolished binding of Tel-2b to the E74 probe.	bind
19482	2	6351	5	NULL	NULL	0	NULL	competitor	NULL	wild-type	abolishes	NULL	completely			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_12_9421_s_308	11108721	10 ng of wild-type competitor completely abolished binding of Tel-2b to the E74 probe.	bind
22553	1	6351	7	NULL	NULL	NULL	NULL	Tel-2b	GP		binds to					E74 probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_12_9421_s_308	11108721	10 ng of wild-type competitor completely abolished binding of Tel-2b to the E74 probe.	bind
22554	2	6351	7	NULL	NULL	NULL	NULL	competitor	GP	wild-type	abolish		completely			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_12_9421_s_308	11108721	10 ng of wild-type competitor completely abolished binding of Tel-2b to the E74 probe.	bind
19483	1	6352	5	NULL	NULL	0	NULL		NULL		bind	NULL		GST DH domain		Cdc42	NULL	recombinant			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_4_1624_s_185	12686614	10 nM GST DH and GST DHPH domains with and without adjacent SH3 domains were bound to recombinant Cdc42 (Figure  4C).	bind
19484	2	6352	5	NULL	NULL	0	NULL	statement 1	NULL		occurs with	NULL					NULL	adjacent	SH3 domains		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_4_1624_s_185	12686614	10 nM GST DH and GST DHPH domains with and without adjacent SH3 domains were bound to recombinant Cdc42 (Figure  4C).	bind
19485	3	6352	5	NULL	NULL	0	NULL	statement 1	NULL		occurs without	NULL					NULL	adjacent	SH3 domains		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_4_1624_s_185	12686614	10 nM GST DH and GST DHPH domains with and without adjacent SH3 domains were bound to recombinant Cdc42 (Figure  4C).	bind
19486	4	6352	5	NULL	NULL	0	NULL		NULL		bind	NULL		GST DHPH domain		Cdc42	NULL	recombinant			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_4_1624_s_185	12686614	10 nM GST DH and GST DHPH domains with and without adjacent SH3 domains were bound to recombinant Cdc42 (Figure  4C).	bind
19487	5	6352	5	NULL	NULL	0	NULL	statement 4	NULL		occurs with	NULL					NULL	adjacent	SH3 domains		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_4_1624_s_185	12686614	10 nM GST DH and GST DHPH domains with and without adjacent SH3 domains were bound to recombinant Cdc42 (Figure  4C).	bind
19488	6	6352	5	NULL	NULL	0	NULL	statement 4	NULL		occurs without	NULL					NULL	adjacent	SH3 domains		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_4_1624_s_185	12686614	10 nM GST DH and GST DHPH domains with and without adjacent SH3 domains were bound to recombinant Cdc42 (Figure  4C).	bind
22555	1	6352	7	NULL	NULL	NULL	NULL				bind			GST DH		Cdc42	GP	recombinant			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_4_1624_s_185	12686614	10 nM GST DH and GST DHPH domains with and without adjacent SH3 domains were bound to recombinant Cdc42 (Figure  4C).	bind
22556	2	6352	7	NULL	NULL	NULL	NULL				bind			 GST DHPH		Cdc42	GP	recombinant			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_4_1624_s_185	12686614	10 nM GST DH and GST DHPH domains with and without adjacent SH3 domains were bound to recombinant Cdc42 (Figure  4C).	bind
22557	3	6352	7	NULL	NULL	0	NULL		NULL		adjacent to	NULL		GST DH			NULL		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_4_1624_s_185	12686614	10 nM GST DH and GST DHPH domains with and without adjacent SH3 domains were bound to recombinant Cdc42 (Figure  4C).	bind
22558	4	6352	7	NULL	NULL	0	NULL		NULL		adjacent to	NULL		GST DHPH			NULL		SH3 domain		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_4_1624_s_185	12686614	10 nM GST DH and GST DHPH domains with and without adjacent SH3 domains were bound to recombinant Cdc42 (Figure  4C).	bind
22559	5	6352	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_4_1624_s_185	12686614	10 nM GST DH and GST DHPH domains with and without adjacent SH3 domains were bound to recombinant Cdc42 (Figure  4C).	bind
22560	6	6352	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs without					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_4_1624_s_185	12686614	10 nM GST DH and GST DHPH domains with and without adjacent SH3 domains were bound to recombinant Cdc42 (Figure  4C).	bind
22561	7	6352	7	NULL	NULL	NULL	NULL	statement 2	Process		occurs with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_4_1624_s_185	12686614	10 nM GST DH and GST DHPH domains with and without adjacent SH3 domains were bound to recombinant Cdc42 (Figure  4C).	bind
22562	8	6352	7	NULL	NULL	NULL	NULL	statement 2	Process		occurs without					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_4_1624_s_185	12686614	10 nM GST DH and GST DHPH domains with and without adjacent SH3 domains were bound to recombinant Cdc42 (Figure  4C).	bind
19489	1	6353	5	NULL	NULL	0	NULL	OHT-ER	NULL		bind	NULL				PI-9 ERU	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_6_5025_s_342	14617632	10 nM OHT induces PI-9 mRNA to levels  20% of those seen with MOX, and OHT-ER binds to the PI-9 ERU roughly 20% as well as MOX-ER.	bind
19490	2	6353	5	NULL	NULL	0	NULL	MOX-ER	NULL		bind	NULL				PI-9 ERU	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_6_5025_s_342	14617632	10 nM OHT induces PI-9 mRNA to levels  20% of those seen with MOX, and OHT-ER binds to the PI-9 ERU roughly 20% as well as MOX-ER.	bind
19491	3	6353	5	NULL	NULL	0	NULL	OHT	NULL		induces	NULL				PI-9 mRNA	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_6_5025_s_342	14617632	10 nM OHT induces PI-9 mRNA to levels  20% of those seen with MOX, and OHT-ER binds to the PI-9 ERU roughly 20% as well as MOX-ER.	bind
19492	4	6353	5	10	NULL	0	NULL	MOX			induces					PI-9 mRNA					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_6_5025_s_342	14617632	10 nM OHT induces PI-9 mRNA to levels  20% of those seen with MOX, and OHT-ER binds to the PI-9 ERU roughly 20% as well as MOX-ER.	bind
22565	1	6353	7	NULL	NULL	NULL	NULL	 OHT	Chemical		induce					PI-9 mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_6_5025_s_342	14617632	10 nM OHT induces PI-9 mRNA to levels  20% of those seen with MOX, and OHT-ER binds to the PI-9 ERU roughly 20% as well as MOX-ER.	bind
22566	2	6353	7	NULL	NULL	NULL	NULL	MOX	Chemical		induce					PI-9 mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_6_5025_s_342	14617632	10 nM OHT induces PI-9 mRNA to levels  20% of those seen with MOX, and OHT-ER binds to the PI-9 ERU roughly 20% as well as MOX-ER.	bind
22567	3	6353	7	NULL	NULL	NULL	NULL	OHT-ER	Chemical		bind					PI-9 ERU	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_6_5025_s_342	14617632	10 nM OHT induces PI-9 mRNA to levels  20% of those seen with MOX, and OHT-ER binds to the PI-9 ERU roughly 20% as well as MOX-ER.	bind
22568	4	6353	7	NULL	NULL	NULL	NULL	MOX-ER	Chemical		bind					PI-9 ERU	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_6_5025_s_342	14617632	10 nM OHT induces PI-9 mRNA to levels  20% of those seen with MOX, and OHT-ER binds to the PI-9 ERU roughly 20% as well as MOX-ER.	bind
19494	1	6354	5	NULL	NULL	0	NULL	growth factors	NULL		promote	NULL				angiogenic function	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_3_462_s_214	11884291	10 Perlecan can bind growth factors that promote angiogenic and tumor growth functions.	bind
19495	2	6354	5	NULL	NULL	0	NULL	growth factors	NULL		promote	NULL				tumor growth function	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_3_462_s_214	11884291	10 Perlecan can bind growth factors that promote angiogenic and tumor growth functions.	bind
19496	3	6354	5	NULL	NULL	0	NULL	Perlecan	NULL		bind	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_3_462_s_214	11884291	10 Perlecan can bind growth factors that promote angiogenic and tumor growth functions.	bind
19497	4	6354	5	NULL	NULL	0	NULL	Perlecan	NULL		bind	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_3_462_s_214	11884291	10 Perlecan can bind growth factors that promote angiogenic and tumor growth functions.	bind
22569	3	6354	7	NULL	NULL	NULL	NULL	Perlecan	Chemical		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_3_462_s_214	11884291	10 Perlecan can bind growth factors that promote angiogenic and tumor growth functions.	bind
22570	1	6354	7	NULL	NULL	NULL	NULL	growth factors	GP		promote					angiogenic function	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_3_462_s_214	11884291	10 Perlecan can bind growth factors that promote angiogenic and tumor growth functions.	bind
22571	2	6354	7	NULL	NULL	NULL	NULL	growth factors	GP		promote					tumor growth function	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_3_462_s_214	11884291	10 Perlecan can bind growth factors that promote angiogenic and tumor growth functions.	bind
29390	4	6354	7	NULL	NULL	NULL	NULL	Perlecan	Chemical		bind					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_3_462_s_214	11884291	10 Perlecan can bind growth factors that promote angiogenic and tumor growth functions.	bind
19498	1	6355	5	NULL	NULL	0	NULL	myosin	NULL		bind	NULL	weakly			actin	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_34_20375_s_8	8702773	10 S cross-linked myosin weakly bound actin (dissociation constant > 500 muM) and did not move actin  in vitro.	bind
19499	2	6355	5	NULL	NULL	0	NULL	myosin	NULL		does not move	NULL				actin	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_271_34_20375_s_8	8702773	10 S cross-linked myosin weakly bound actin (dissociation constant > 500 muM) and did not move actin  in vitro.	bind
22572	1	6355	7	NULL	NULL	NULL	NULL	myosin	GP	S cross-linked	bind		weakly			actin	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_34_20375_s_8	8702773	10 S cross-linked myosin weakly bound actin (dissociation constant > 500 muM) and did not move actin  in vitro.	bind
22573	2	6355	7	NULL	NULL	NULL	NULL	myosin	GP	S cross-linked	does not move					actin	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_34_20375_s_8	8702773	10 S cross-linked myosin weakly bound actin (dissociation constant > 500 muM) and did not move actin  in vitro.	bind
19500	1	6356	5	10	NULL	0	NULL	nuclear protein			bind									NF-kappaB sequences	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1414_s_196	11557665	10 Similarly, LDL treatment appears to have little effect on the nuclear protein binding to the ICAM-1 - specific NF-kappaB sequences.	bind
19501	2	6356	5	10	NULL	0	NULL	LDL		treatment	effects		negligibly			statement 1					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1414_s_196	11557665	10 Similarly, LDL treatment appears to have little effect on the nuclear protein binding to the ICAM-1 - specific NF-kappaB sequences.	bind
54215	3	6356	5	10	NULL	0	NULL				is specific to				NF-kappaB sequences	ICAM-1					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1414_s_196	11557665	10 Similarly, LDL treatment appears to have little effect on the nuclear protein binding to the ICAM-1 - specific NF-kappaB sequences.	bind
22574	1	6356	7	NULL	NULL	NULL	NULL	nuclear protein	GP		bind									NF-kappaB sequence	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1414_s_196	11557665	10 Similarly, LDL treatment appears to have little effect on the nuclear protein binding to the ICAM-1 - specific NF-kappaB sequences.	bind
22575	2	6356	7	NULL	NULL	NULL	NULL				is specific to				NF-kappaB sequence	ICAM-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1414_s_196	11557665	10 Similarly, LDL treatment appears to have little effect on the nuclear protein binding to the ICAM-1 - specific NF-kappaB sequences.	bind
22576	3	6356	7	NULL	NULL	NULL	NULL	LDL	GP	treatment	effect		negligibly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1414_s_196	11557665	10 Similarly, LDL treatment appears to have little effect on the nuclear protein binding to the ICAM-1 - specific NF-kappaB sequences.	bind
19502	1	6357	5	NULL	NULL	0	NULL	Sp3	NULL		bind	NULL					NULL			GC box	NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_907_s_168	12067897	10 Sp3 is bound to a GC box with an affinity and specificity comparable to those of Sp1 and, thereby, represses Sp1-mediated transcription.	bind
19503	3	6357	5	NULL	NULL	0	NULL	statement 1	NULL	affinity of	is comparable to	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_907_s_168	12067897	10 Sp3 is bound to a GC box with an affinity and specificity comparable to those of Sp1 and, thereby, represses Sp1-mediated transcription.	bind
19504	4	6357	5	NULL	NULL	0	NULL	statement 1	NULL	specificity of	is comparable to	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_907_s_168	12067897	10 Sp3 is bound to a GC box with an affinity and specificity comparable to those of Sp1 and, thereby, represses Sp1-mediated transcription.	bind
19505	5	6357	5	10	NULL	0	NULL	Sp1			mediate					transcription					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_907_s_168	12067897	10 Sp3 is bound to a GC box with an affinity and specificity comparable to those of Sp1 and, thereby, represses Sp1-mediated transcription.	bind
19506	6	6357	5	10	NULL	0	NULL	statement 1			repress					statement 5					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_907_s_168	12067897	10 Sp3 is bound to a GC box with an affinity and specificity comparable to those of Sp1 and, thereby, represses Sp1-mediated transcription.	bind
23074	2	6357	5	NULL	NULL	0	NULL	Sp1	NULL		bind	NULL					NULL			GC box	NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_907_s_168	12067897	10 Sp3 is bound to a GC box with an affinity and specificity comparable to those of Sp1 and, thereby, represses Sp1-mediated transcription.	bind
22577	1	6357	7	NULL	NULL	NULL	NULL	 Sp3	GP		bind									GC box	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_907_s_168	12067897	10 Sp3 is bound to a GC box with an affinity and specificity comparable to those of Sp1 and, thereby, represses Sp1-mediated transcription.	bind
22578	2	6357	7	NULL	NULL	NULL	NULL	Sp1	GP		bind									GC box	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_907_s_168	12067897	10 Sp3 is bound to a GC box with an affinity and specificity comparable to those of Sp1 and, thereby, represses Sp1-mediated transcription.	bind
22579	3	6357	7	NULL	NULL	NULL	NULL	statement 1	Process	affinity of	is comparable to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_907_s_168	12067897	10 Sp3 is bound to a GC box with an affinity and specificity comparable to those of Sp1 and, thereby, represses Sp1-mediated transcription.	bind
22580	5	6357	7	NULL	NULL	NULL	NULL	Sp1	GP		mediates					transcription	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_907_s_168	12067897	10 Sp3 is bound to a GC box with an affinity and specificity comparable to those of Sp1 and, thereby, represses Sp1-mediated transcription.	bind
22581	6	6357	7	NULL	NULL	NULL	NULL	statement 1	Process		repress					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_907_s_168	12067897	10 Sp3 is bound to a GC box with an affinity and specificity comparable to those of Sp1 and, thereby, represses Sp1-mediated transcription.	bind
22981	4	6357	7	NULL	NULL	NULL	NULL	statement 1	Process	specificity of	is comparable to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_907_s_168	12067897	10 Sp3 is bound to a GC box with an affinity and specificity comparable to those of Sp1 and, thereby, represses Sp1-mediated transcription.	bind
19507	1	6358	5	NULL	NULL	0	NULL	ERalpha	NULL		bind	NULL				target genes	NULL			estrogen-responsive promoters	NULL		0	NULL	NULL	NULL	gw60_circulation_105_22_2653_s_30	12045172	10 SRC-3 was recently shown to be associated with ERalpha bound to the estrogen-responsive promoters of target genes after estrogen treatment.	bind
19508	2	6358	5	NULL	NULL	0	NULL	SRC-3	NULL		is associated with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_22_2653_s_30	12045172	10 SRC-3 was recently shown to be associated with ERalpha bound to the estrogen-responsive promoters of target genes after estrogen treatment.	bind
19509	3	6358	5	NULL	NULL	0	NULL	statement 2	NULL		occurs after	NULL				estrogen	NULL	treatment			NULL		0	NULL	NULL	NULL	gw60_circulation_105_22_2653_s_30	12045172	10 SRC-3 was recently shown to be associated with ERalpha bound to the estrogen-responsive promoters of target genes after estrogen treatment.	bind
22634	1	6358	7	NULL	NULL	NULL	NULL	ERalpha 	GP		bind									estrogen-responsive promoter	NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_22_2653_s_30	12045172	10 SRC-3 was recently shown to be associated with ERalpha bound to the estrogen-responsive promoters of target genes after estrogen treatment.	bind
22635	3	6358	7	NULL	NULL	NULL	NULL	statement 2	Process		occurs after					estrogen	GP	treatment			NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_22_2653_s_30	12045172	10 SRC-3 was recently shown to be associated with ERalpha bound to the estrogen-responsive promoters of target genes after estrogen treatment.	bind
22636	2	6358	7	NULL	NULL	NULL	NULL	SRC-3	GP		associate with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_22_2653_s_30	12045172	10 SRC-3 was recently shown to be associated with ERalpha bound to the estrogen-responsive promoters of target genes after estrogen treatment.	bind
19510	1	6359	5	NULL	NULL	0	NULL	FKBP12.6	NULL		does not bind	NULL				RyR2	NULL	phosphorylated	serine-2808		NULL		0	NULL	NULL	NULL	gw70_circulationres_94_4_487_s_26	14715536	10 These observations have led to the notions that FKBP12.6 cannot bind to serine-2808 phosphorylated RyR2 and that PKA phosphorylation physiologically regulates FKBP12.6-RyR2 interaction.	bind
19511	2	6359	5	10	NULL	0	NULL	PKA	NULL	phosphorylation	regulates	NULL	physiologically			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_4_487_s_26	14715536	10 These observations have led to the notions that FKBP12.6 cannot bind to serine-2808 phosphorylated RyR2 and that PKA phosphorylation physiologically regulates FKBP12.6-RyR2 interaction.	bind
22637	1	6359	7	NULL	NULL	NULL	NULL	FKBP12.6	GP		does not bind					RyR2	GP	phosphorylated	serine-2808		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_4_487_s_26	14715536	10 These observations have led to the notions that FKBP12.6 cannot bind to serine-2808 phosphorylated RyR2 and that PKA phosphorylation physiologically regulates FKBP12.6-RyR2 interaction.	bind
22638	2	6359	7	NULL	NULL	NULL	NULL	PKA	GP	phosphorylation of	regulates		physiologically			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_4_487_s_26	14715536	10 These observations have led to the notions that FKBP12.6 cannot bind to serine-2808 phosphorylated RyR2 and that PKA phosphorylation physiologically regulates FKBP12.6-RyR2 interaction.	bind
19512	1	6361	5	NULL	NULL	0	NULL	FKBP12.6	NULL		bind	NULL				RyR2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_4_487_s_225	14715536	10 This is surprising, given our previous observation that a large region in RyR2 (residues 1937 to 4967) encompassing the serine-2808 phosphorylation site and the previously mapped FKBP12.6 binding site (residues 2427 through 2428) is not required for FKBP12.6 binding to RyR2.	bind
19513	2	6361	5	10	NULL	0	NULL	RyR2			encompass			\tresidues 1937 to 4967					serine-2808 phosphorylation site		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_4_487_s_225	14715536	10 This is surprising, given our previous observation that a large region in RyR2 (residues 1937 to 4967) encompassing the serine-2808 phosphorylation site and the previously mapped FKBP12.6 binding site (residues 2427 through 2428) is not required for FKBP12.6 binding to RyR2.	bind
19514	3	6361	5	10	NULL	0	NULL	RyR2			encompass			residues 2427 through 2428					FKBP12.6 binding site		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_4_487_s_225	14715536	10 This is surprising, given our previous observation that a large region in RyR2 (residues 1937 to 4967) encompassing the serine-2808 phosphorylation site and the previously mapped FKBP12.6 binding site (residues 2427 through 2428) is not required for FKBP12.6 binding to RyR2.	bind
19515	4	6361	5	NULL	NULL	0	NULL	statement 1	NULL		does not require	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_4_487_s_225	14715536	10 This is surprising, given our previous observation that a large region in RyR2 (residues 1937 to 4967) encompassing the serine-2808 phosphorylation site and the previously mapped FKBP12.6 binding site (residues 2427 through 2428) is not required for FKBP12.6 binding to RyR2.	bind
19516	5	6361	5	NULL	NULL	0	NULL	statement 1	NULL		does not require	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_4_487_s_225	14715536	10 This is surprising, given our previous observation that a large region in RyR2 (residues 1937 to 4967) encompassing the serine-2808 phosphorylation site and the previously mapped FKBP12.6 binding site (residues 2427 through 2428) is not required for FKBP12.6 binding to RyR2.	bind
22639	1	6361	7	NULL	NULL	NULL	NULL	FKBP12.6	GP		bind					RyR2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_4_487_s_225	14715536	10 This is surprising, given our previous observation that a large region in RyR2 (residues 1937 to 4967) encompassing the serine-2808 phosphorylation site and the previously mapped FKBP12.6 binding site (residues 2427 through 2428) is not required for FKBP12.6 binding to RyR2.	bind
22640	2	6361	7	NULL	NULL	NULL	NULL	RyR2	GP		encompass			residues 1937 to 4967					serine-2808 phosphorylation site		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_4_487_s_225	14715536	10 This is surprising, given our previous observation that a large region in RyR2 (residues 1937 to 4967) encompassing the serine-2808 phosphorylation site and the previously mapped FKBP12.6 binding site (residues 2427 through 2428) is not required for FKBP12.6 binding to RyR2.	bind
22641	3	6361	7	NULL	NULL	NULL	NULL	RyR2	GP		encompass			residues 2427 through 2428					FKBP12.6 binding site		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_4_487_s_225	14715536	10 This is surprising, given our previous observation that a large region in RyR2 (residues 1937 to 4967) encompassing the serine-2808 phosphorylation site and the previously mapped FKBP12.6 binding site (residues 2427 through 2428) is not required for FKBP12.6 binding to RyR2.	bind
22642	4	6361	7	NULL	NULL	NULL	NULL	statement 2	Process		is not required for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_4_487_s_225	14715536	10 This is surprising, given our previous observation that a large region in RyR2 (residues 1937 to 4967) encompassing the serine-2808 phosphorylation site and the previously mapped FKBP12.6 binding site (residues 2427 through 2428) is not required for FKBP12.6 binding to RyR2.	bind
54216	5	6361	7	NULL	NULL	NULL	NULL	statement 3	Process		is not required for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_4_487_s_225	14715536	10 This is surprising, given our previous observation that a large region in RyR2 (residues 1937 to 4967) encompassing the serine-2808 phosphorylation site and the previously mapped FKBP12.6 binding site (residues 2427 through 2428) is not required for FKBP12.6 binding to RyR2.	bind
19517	1	6362	5	NULL	NULL	0	NULL	VEGF	NULL		bind	NULL				VEGFR-1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_11_1443_s_22	15192038	10 VEGF binds to VEGFR-1 and VEGFR-2 and induces vasculogenesis, angiogenesis, and vascular permeability.	bind
19518	2	6362	5	NULL	NULL	0	NULL	VEGF	NULL		bind	NULL				VEGFR-2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_11_1443_s_22	15192038	10 VEGF binds to VEGFR-1 and VEGFR-2 and induces vasculogenesis, angiogenesis, and vascular permeability.	bind
19519	3	6362	5	NULL	NULL	0	NULL	VEGF	NULL		induces	NULL				vasculogenesis	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_11_1443_s_22	15192038	10 VEGF binds to VEGFR-1 and VEGFR-2 and induces vasculogenesis, angiogenesis, and vascular permeability.	bind
19520	4	6362	5	NULL	NULL	0	NULL	VEGF	NULL		induces	NULL				angiogenesis	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_11_1443_s_22	15192038	10 VEGF binds to VEGFR-1 and VEGFR-2 and induces vasculogenesis, angiogenesis, and vascular permeability.	bind
19521	5	6362	5	NULL	NULL	0	NULL	VEGF	NULL		induces	NULL				vascular permeability	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_11_1443_s_22	15192038	10 VEGF binds to VEGFR-1 and VEGFR-2 and induces vasculogenesis, angiogenesis, and vascular permeability.	bind
22643	1	6362	7	NULL	NULL	NULL	NULL	VEGF	GP		binds					 VEGFR-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1443_s_22	15192038	10 VEGF binds to VEGFR-1 and VEGFR-2 and induces vasculogenesis, angiogenesis, and vascular permeability.	bind
22644	2	6362	7	NULL	NULL	NULL	NULL	VEGF	GP		binds					VEGFR-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1443_s_22	15192038	10 VEGF binds to VEGFR-1 and VEGFR-2 and induces vasculogenesis, angiogenesis, and vascular permeability.	bind
22645	3	6362	7	NULL	NULL	NULL	NULL	statement 1	Process		induces					vasculogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1443_s_22	15192038	10 VEGF binds to VEGFR-1 and VEGFR-2 and induces vasculogenesis, angiogenesis, and vascular permeability.	bind
22646	4	6362	7	NULL	NULL	NULL	NULL	statement 1	Process		induces					angiogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1443_s_22	15192038	10 VEGF binds to VEGFR-1 and VEGFR-2 and induces vasculogenesis, angiogenesis, and vascular permeability.	bind
22647	5	6362	7	NULL	NULL	NULL	NULL	statement 1	Process		induces					vascular permeability	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1443_s_22	15192038	10 VEGF binds to VEGFR-1 and VEGFR-2 and induces vasculogenesis, angiogenesis, and vascular permeability.	bind
22648	6	6362	7	NULL	NULL	NULL	NULL	statement 2	Process		induces					vasculogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1443_s_22	15192038	10 VEGF binds to VEGFR-1 and VEGFR-2 and induces vasculogenesis, angiogenesis, and vascular permeability.	bind
22649	7	6362	7	NULL	NULL	NULL	NULL	statement 2	Process		induces					angiogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1443_s_22	15192038	10 VEGF binds to VEGFR-1 and VEGFR-2 and induces vasculogenesis, angiogenesis, and vascular permeability.	bind
22650	8	6362	7	NULL	NULL	NULL	NULL	statement 2	Process		induces					vascular permeability	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1443_s_22	15192038	10 VEGF binds to VEGFR-1 and VEGFR-2 and induces vasculogenesis, angiogenesis, and vascular permeability.	bind
19522	1	6363	5	NULL	NULL	0	NULL	[ H]LPS	NULL		bind	NULL	significantly			CD14	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_361_s_35	7529231	10%  human serum was required for  significant [ H]LPS binding to CD14.	bind
19523	2	6363	5	NULL	NULL	0	NULL	serum	NULL	human	is required for	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_361_s_35	7529231	10%  human serum was required for  significant [ H]LPS binding to CD14.	bind
22651	1	6363	7	NULL	NULL	NULL	NULL	[ H]LPS	Chemical		bind					CD14	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_361_s_35	7529231	10%  human serum was required for  significant [ H]LPS binding to CD14.	bind
22652	2	6363	7	NULL	NULL	NULL	NULL	serum	OrganismPart	human	is required for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_361_s_35	7529231	10%  human serum was required for  significant [ H]LPS binding to CD14.	bind
19524	1	6364	5	NULL	NULL	0	NULL	betabeta receptor dimer	NULL		bind	NULL				PDGF-BB	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_6_1763_s_17	10362801	10, 11 The betabeta receptor dimer binds only PDGF-BB, the alphabeta receptor dimer binds PDGF-BB and PDGF-AB, and the alphaalpha receptor dimer binds all three types of PDGF dimers.	bind
19525	2	6364	5	NULL	NULL	0	NULL	alphabeta receptor dimer	NULL		bind	NULL				PDGF-BB	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_6_1763_s_17	10362801	10, 11 The betabeta receptor dimer binds only PDGF-BB, the alphabeta receptor dimer binds PDGF-BB and PDGF-AB, and the alphaalpha receptor dimer binds all three types of PDGF dimers.	bind
19526	3	6364	5	NULL	NULL	0	NULL	alphabeta receptor dimer	NULL		bind	NULL				PDGF-AB	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_6_1763_s_17	10362801	10, 11 The betabeta receptor dimer binds only PDGF-BB, the alphabeta receptor dimer binds PDGF-BB and PDGF-AB, and the alphaalpha receptor dimer binds all three types of PDGF dimers.	bind
19527	4	6364	5	10	NULL	0	NULL	alphaalpha receptor dimer	NULL		bind	NULL				PDGF-AB	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1763_s_17	10362801	10, 11 The betabeta receptor dimer binds only PDGF-BB, the alphabeta receptor dimer binds PDGF-BB and PDGF-AB, and the alphaalpha receptor dimer binds all three types of PDGF dimers.	bind
54217	5	6364	5	10	NULL	0	NULL	alphaalpha receptor dimer			bind					PDGF-BB					NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_6_1763_s_17	10362801	10, 11 The betabeta receptor dimer binds only PDGF-BB, the alphabeta receptor dimer binds PDGF-BB and PDGF-AB, and the alphaalpha receptor dimer binds all three types of PDGF dimers.	bind
22653	1	6364	7	NULL	NULL	NULL	NULL	betabeta receptor dimer	GP		binds					PDGF-BB	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1763_s_17	10362801	10, 11 The betabeta receptor dimer binds only PDGF-BB, the alphabeta receptor dimer binds PDGF-BB and PDGF-AB, and the alphaalpha receptor dimer binds all three types of PDGF dimers.	bind
22654	2	6364	7	NULL	NULL	NULL	NULL	alphabeta receptor dimer 	GP		binds					PDGF-BB	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1763_s_17	10362801	10, 11 The betabeta receptor dimer binds only PDGF-BB, the alphabeta receptor dimer binds PDGF-BB and PDGF-AB, and the alphaalpha receptor dimer binds all three types of PDGF dimers.	bind
22655	3	6364	7	NULL	NULL	NULL	NULL	alphabeta receptor dimer 	GP		binds					PDGF-AB	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1763_s_17	10362801	10, 11 The betabeta receptor dimer binds only PDGF-BB, the alphabeta receptor dimer binds PDGF-BB and PDGF-AB, and the alphaalpha receptor dimer binds all three types of PDGF dimers.	bind
22656	4	6364	7	NULL	NULL	NULL	NULL	alphaalpha receptor dimer	GP		binds					PDGF-BB	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1763_s_17	10362801	10, 11 The betabeta receptor dimer binds only PDGF-BB, the alphabeta receptor dimer binds PDGF-BB and PDGF-AB, and the alphaalpha receptor dimer binds all three types of PDGF dimers.	bind
22657	5	6364	7	NULL	NULL	NULL	NULL	alphaalpha receptor dimer	GP		binds					PDGF-AB	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1763_s_17	10362801	10, 11 The betabeta receptor dimer binds only PDGF-BB, the alphabeta receptor dimer binds PDGF-BB and PDGF-AB, and the alphaalpha receptor dimer binds all three types of PDGF dimers.	bind
23075	1	6365	5	NULL	NULL	0	NULL	cMyBP-C	NULL		undergoes	NULL				trimerization	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_9_1249_s_19	15059932	10,11  It has been proposed that cMyBP-C trimerizes to form a collar around the thick filament 2,3,7   with interdomain binding of C5 and C7 of one molecule to C8 and C10, respectively, of another.	bind
23076	2	6365	5	NULL	NULL	0	NULL	statement 1	NULL		forms	NULL				collar	NULL				NULL	around thick filament	0	NULL	NULL	NULL	gw70_circulationres_94_9_1249_s_19	15059932	10,11  It has been proposed that cMyBP-C trimerizes to form a collar around the thick filament 2,3,7   with interdomain binding of C5 and C7 of one molecule to C8 and C10, respectively, of another.	bind
23077	3	6365	5	NULL	NULL	0	NULL	myosin binding protein-C	NULL	interdomains of	bind	NULL		C5		myosin binding protein-C	NULL		C8		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_9_1249_s_19	15059932	10,11  It has been proposed that cMyBP-C trimerizes to form a collar around the thick filament 2,3,7   with interdomain binding of C5 and C7 of one molecule to C8 and C10, respectively, of another.	bind
23078	4	6365	5	NULL	NULL	0	NULL	myosin binding protein-C	NULL	interdomains of	bind	NULL		C7		myosin binding protein-C	NULL		C10		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_9_1249_s_19	15059932	10,11  It has been proposed that cMyBP-C trimerizes to form a collar around the thick filament 2,3,7   with interdomain binding of C5 and C7 of one molecule to C8 and C10, respectively, of another.	bind
22658	1	6365	7	NULL	NULL	NULL	NULL	cMyBP-C	GP		undergoes					trimerization	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_9_1249_s_19	15059932	10,11  It has been proposed that cMyBP-C trimerizes to form a collar around the thick filament 2,3,7   with interdomain binding of C5 and C7 of one molecule to C8 and C10, respectively, of another.	bind
22659	3	6365	7	NULL	NULL	NULL	NULL	cMyBP-C	GP	interdomain	binds to			C5 		cMyBP-C	GP	interdomain	C8		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_9_1249_s_19	15059932	10,11  It has been proposed that cMyBP-C trimerizes to form a collar around the thick filament 2,3,7   with interdomain binding of C5 and C7 of one molecule to C8 and C10, respectively, of another.	bind
22660	4	6365	7	NULL	NULL	NULL	NULL	cMyBP-C	GP	interdomain	binds to			C7		cMyBP-C	GP	interdomain	C10		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_9_1249_s_19	15059932	10,11  It has been proposed that cMyBP-C trimerizes to form a collar around the thick filament 2,3,7   with interdomain binding of C5 and C7 of one molecule to C8 and C10, respectively, of another.	bind
29391	2	6365	7	NULL	NULL	NULL	NULL	statement 1	Process		forms					collar	OrganismPart				NULL	around thick filament	NULL	NULL	NULL	NULL	gw70_circulationres_94_9_1249_s_19	15059932	10,11  It has been proposed that cMyBP-C trimerizes to form a collar around the thick filament 2,3,7   with interdomain binding of C5 and C7 of one molecule to C8 and C10, respectively, of another.	bind
19619	1	6370	5	NULL	NULL	0	NULL	estrogen receptor	NULL	human	bind	NULL					NULL			estrogen response element	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_597	11452016	100       Nardulli,A.M., Greene,G.L. and Shapiro,D.J. (1993) Human estrogen receptor bound to an estrogen response element bends DNA.	bind
19620	2	6370	5	NULL	NULL	0	NULL	statement 1	NULL		bends	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_597	11452016	100       Nardulli,A.M., Greene,G.L. and Shapiro,D.J. (1993) Human estrogen receptor bound to an estrogen response element bends DNA.	bind
22661	1	6370	7	NULL	NULL	NULL	NULL	estrogen receptor	GP	human	binds to									estrogen response element 	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_597	11452016	100       Nardulli,A.M., Greene,G.L. and Shapiro,D.J. (1993) Human estrogen receptor bound to an estrogen response element bends DNA.	bind
22662	2	6370	7	NULL	NULL	NULL	NULL	statement 1	Process		bends 					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_597	11452016	100       Nardulli,A.M., Greene,G.L. and Shapiro,D.J. (1993) Human estrogen receptor bound to an estrogen response element bends DNA.	bind
23079	1	6375	5	NULL	NULL	0	NULL	[3]ALDO	NULL		bind	NULL				surface	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_98_1_157_s_4	8690788	100 nM 8-Br-cGMP decreased  surface [3]ALDO binding by 42 plus-or-minus 4% but increased crypt  [3]ALDO binding by 52 plus-or-minus 16%.	bind
23080	2	6375	5	NULL	NULL	0	NULL	[3]ALDO	NULL		bind	NULL				crypt	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_98_1_157_s_4	8690788	100 nM 8-Br-cGMP decreased  surface [3]ALDO binding by 42 plus-or-minus 4% but increased crypt  [3]ALDO binding by 52 plus-or-minus 16%.	bind
28697	3	6375	5	NULL	NULL	0	NULL	8-Br-cGMP	NULL		decreases	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_98_1_157_s_4	8690788	100 nM 8-Br-cGMP decreased  surface [3]ALDO binding by 42 plus-or-minus 4% but increased crypt  [3]ALDO binding by 52 plus-or-minus 16%.	bind
28698	4	6375	5	NULL	NULL	0	NULL	8-Br-cGMP	NULL		increases	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_98_1_157_s_4	8690788	100 nM 8-Br-cGMP decreased  surface [3]ALDO binding by 42 plus-or-minus 4% but increased crypt  [3]ALDO binding by 52 plus-or-minus 16%.	bind
22713	1	6375	7	NULL	NULL	NULL	NULL	[3]ALDO	Chemical		bind					surface	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_98_1_157_s_4	8690788	100 nM 8-Br-cGMP decreased  surface [3]ALDO binding by 42 plus-or-minus 4% but increased crypt  [3]ALDO binding by 52 plus-or-minus 16%.	bind
22714	2	6375	7	NULL	NULL	NULL	NULL	 [3]ALDO	Chemical		bind					crypt	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_98_1_157_s_4	8690788	100 nM 8-Br-cGMP decreased  surface [3]ALDO binding by 42 plus-or-minus 4% but increased crypt  [3]ALDO binding by 52 plus-or-minus 16%.	bind
22715	3	6375	7	NULL	NULL	NULL	NULL	 8-Br-cGMP 	Chemical		decrease					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_98_1_157_s_4	8690788	100 nM 8-Br-cGMP decreased  surface [3]ALDO binding by 42 plus-or-minus 4% but increased crypt  [3]ALDO binding by 52 plus-or-minus 16%.	bind
22716	4	6375	7	NULL	NULL	NULL	NULL	 8-Br-cGMP 	Chemical		increase					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_98_1_157_s_4	8690788	100 nM 8-Br-cGMP decreased  surface [3]ALDO binding by 42 plus-or-minus 4% but increased crypt  [3]ALDO binding by 52 plus-or-minus 16%.	bind
19621	1	6378	5	10	NULL	0	NULL	Hsc70			bind					clathrin			heavy chain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_12_8439_s_227	10722678	100% complex indicates one Hsc70 bound per clathrin heavy chain in the reaction mixture.	bind
22718	1	6378	7	NULL	NULL	NULL	NULL	Hsc70	GP		bind					clathrin	GP		heavy chain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_12_8439_s_227	10722678	100% complex indicates one Hsc70 bound per clathrin heavy chain in the reaction mixture.	bind
19622	1	6379	5	NULL	NULL	0	NULL	[gamma-32]GTP	NULL		bind	NULL				Arf1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_11_10128_s_244	15644318	100% refers the amount of [gamma-32]GTP bound to Arf1 or RhoA in the absence of M9b-tail.	bind
19623	2	6379	5	NULL	NULL	0	NULL	statement 1	NULL		in the absence of	NULL				M9b-tail	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_11_10128_s_244	15644318	100% refers the amount of [gamma-32]GTP bound to Arf1 or RhoA in the absence of M9b-tail.	bind
19624	3	6379	5	NULL	NULL	0	NULL	[gamma-32]GTP	NULL		bind	NULL				RhoA	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_11_10128_s_244	15644318	100% refers the amount of [gamma-32]GTP bound to Arf1 or RhoA in the absence of M9b-tail.	bind
19625	4	6379	5	NULL	NULL	0	NULL	statement 3	NULL		in the absence of	NULL				M9b-tail	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_11_10128_s_244	15644318	100% refers the amount of [gamma-32]GTP bound to Arf1 or RhoA in the absence of M9b-tail.	bind
19626	5	6379	5	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_11_10128_s_244	15644318	100% refers the amount of [gamma-32]GTP bound to Arf1 or RhoA in the absence of M9b-tail.	bind
22720	1	6379	7	NULL	NULL	NULL	NULL	[gamma-32]GTP 	Chemical		bind					Arf1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_10128_s_244	15644318	100% refers the amount of [gamma-32]GTP bound to Arf1 or RhoA in the absence of M9b-tail.	bind
22722	2	6379	7	NULL	NULL	NULL	NULL	[gamma-32]GTP	Chemical		bind					RhoA 	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_10128_s_244	15644318	100% refers the amount of [gamma-32]GTP bound to Arf1 or RhoA in the absence of M9b-tail.	bind
22723	3	6379	7	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_10128_s_244	15644318	100% refers the amount of [gamma-32]GTP bound to Arf1 or RhoA in the absence of M9b-tail.	bind
22725	4	6379	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs in absence of					M9b-tail	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_10128_s_244	15644318	100% refers the amount of [gamma-32]GTP bound to Arf1 or RhoA in the absence of M9b-tail.	bind
22726	5	6379	7	NULL	NULL	NULL	NULL	statement 2	Process		occurs in  absence of					M9b-tail	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_10128_s_244	15644318	100% refers the amount of [gamma-32]GTP bound to Arf1 or RhoA in the absence of M9b-tail.	bind
19627	1	6380	5	NULL	NULL	0	NULL	VEGF	NULL		bind	NULL				alpha2M-MA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_35_26806_s_140	10862607	100% represents total VEGF bound to either alpha2M-MA or alpha2M-PPE.	bind
19628	2	6380	5	NULL	NULL	0	NULL	VEGF	NULL		bind	NULL				alpha2M-PPE	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_35_26806_s_140	10862607	100% represents total VEGF bound to either alpha2M-MA or alpha2M-PPE.	bind
19629	3	6380	5	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_35_26806_s_140	10862607	100% represents total VEGF bound to either alpha2M-MA or alpha2M-PPE.	bind
22732	1	6380	7	NULL	NULL	NULL	NULL	VEGF	GP		bind					alpha2M-MA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_35_26806_s_140	10862607	100% represents total VEGF bound to either alpha2M-MA or alpha2M-PPE.	bind
22733	2	6380	7	NULL	NULL	NULL	NULL	VEGF	GP		bind					alpha2M-PPE	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_35_26806_s_140	10862607	100% represents total VEGF bound to either alpha2M-MA or alpha2M-PPE.	bind
29394	3	6380	7	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_35_26806_s_140	10862607	100% represents total VEGF bound to either alpha2M-MA or alpha2M-PPE.	bind
19630	1	6381	5	NULL	NULL	0	NULL	HSP	NULL		bind	NULL				HIF-1beta/ARNT	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_1_15_s_188	15637304	100,101  HSP binding to HIF-1beta/ARNT acts as a chaperone, maintaining HIF-1alpha in a receptive state for signaling.	bind
19631	2	6381	5	NULL	NULL	0	NULL	statement 1	NULL		acts as	NULL				chaperone	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_1_15_s_188	15637304	100,101  HSP binding to HIF-1beta/ARNT acts as a chaperone, maintaining HIF-1alpha in a receptive state for signaling.	bind
19632	3	6381	5	10	NULL	0	NULL	HIF-1alpha	NULL		is maintained in	NULL				receptive state	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_1_15_s_188	15637304	100,101  HSP binding to HIF-1beta/ARNT acts as a chaperone, maintaining HIF-1alpha in a receptive state for signaling.	bind
19633	4	6381	5	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_1_15_s_188	15637304	100,101  HSP binding to HIF-1beta/ARNT acts as a chaperone, maintaining HIF-1alpha in a receptive state for signaling.	bind
22735	1	6381	7	NULL	NULL	NULL	NULL	HSP	GP		bind					HIF-1beta/ARNT	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_1_15_s_188	15637304	100,101  HSP binding to HIF-1beta/ARNT acts as a chaperone, maintaining HIF-1alpha in a receptive state for signaling.	bind
22736	2	6381	7	NULL	NULL	NULL	NULL	statement 1	Process		acts as a					chaperone	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_1_15_s_188	15637304	100,101  HSP binding to HIF-1beta/ARNT acts as a chaperone, maintaining HIF-1alpha in a receptive state for signaling.	bind
22737	3	6381	7	NULL	NULL	NULL	NULL	HIF-1 alpha	GP		is maintained at					receptive state	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_1_15_s_188	15637304	100,101  HSP binding to HIF-1beta/ARNT acts as a chaperone, maintaining HIF-1alpha in a receptive state for signaling.	bind
23081	1	6382	5	NULL	NULL	0	NULL	SR-BI	NULL		mediate	NULL				cholesterol efflux	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_13_s_150	11145929	102  However, SR-BI - mediated cholesterol efflux does not simply reflect the binding of HDL to cells, inasmuch as binding of HDL to CD36, which is another HDL binding scavenger receptor, does not facilitate cholesterol efflux.	bind
23082	2	6382	5	NULL	NULL	0	NULL	HDL	NULL		bind	NULL				cells	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_13_s_150	11145929	102  However, SR-BI - mediated cholesterol efflux does not simply reflect the binding of HDL to cells, inasmuch as binding of HDL to CD36, which is another HDL binding scavenger receptor, does not facilitate cholesterol efflux.	bind
23083	3	6382	5	NULL	NULL	0	NULL	statement 1	NULL		reflects	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_13_s_150	11145929	102  However, SR-BI - mediated cholesterol efflux does not simply reflect the binding of HDL to cells, inasmuch as binding of HDL to CD36, which is another HDL binding scavenger receptor, does not facilitate cholesterol efflux.	bind
23084	4	6382	5	NULL	NULL	0	NULL	HDL	NULL		bind	NULL				CD36	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_13_s_150	11145929	102  However, SR-BI - mediated cholesterol efflux does not simply reflect the binding of HDL to cells, inasmuch as binding of HDL to CD36, which is another HDL binding scavenger receptor, does not facilitate cholesterol efflux.	bind
23085	5	6382	5	NULL	NULL	0	NULL	CD36	NULL		is	NULL				HDL binding scavenger receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_13_s_150	11145929	102  However, SR-BI - mediated cholesterol efflux does not simply reflect the binding of HDL to cells, inasmuch as binding of HDL to CD36, which is another HDL binding scavenger receptor, does not facilitate cholesterol efflux.	bind
23086	6	6382	5	NULL	NULL	0	NULL	statement 4	NULL		does not facilitate	NULL				cholesterol efflux	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_13_s_150	11145929	102  However, SR-BI - mediated cholesterol efflux does not simply reflect the binding of HDL to cells, inasmuch as binding of HDL to CD36, which is another HDL binding scavenger receptor, does not facilitate cholesterol efflux.	bind
22738	1	6382	7	NULL	NULL	NULL	NULL	HDL	GP		bind					cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_13_s_150	11145929	102  However, SR-BI - mediated cholesterol efflux does not simply reflect the binding of HDL to cells, inasmuch as binding of HDL to CD36, which is another HDL binding scavenger receptor, does not facilitate cholesterol efflux.	bind
22739	2	6382	7	NULL	NULL	NULL	NULL	HDL	GP		bind					CD36	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_13_s_150	11145929	102  However, SR-BI - mediated cholesterol efflux does not simply reflect the binding of HDL to cells, inasmuch as binding of HDL to CD36, which is another HDL binding scavenger receptor, does not facilitate cholesterol efflux.	bind
22740	3	6382	7	NULL	NULL	NULL	NULL	SR-BI	Cell		mediates					cholesterol 	Chemical	efflux of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_13_s_150	11145929	102  However, SR-BI - mediated cholesterol efflux does not simply reflect the binding of HDL to cells, inasmuch as binding of HDL to CD36, which is another HDL binding scavenger receptor, does not facilitate cholesterol efflux.	bind
22743	4	6382	7	NULL	NULL	NULL	NULL	statement 3	Process		does not reflect					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_13_s_150	11145929	102  However, SR-BI - mediated cholesterol efflux does not simply reflect the binding of HDL to cells, inasmuch as binding of HDL to CD36, which is another HDL binding scavenger receptor, does not facilitate cholesterol efflux.	bind
22745	5	6382	7	NULL	NULL	NULL	NULL	CD36	Cell		is					HDL binding scavenger receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_13_s_150	11145929	102  However, SR-BI - mediated cholesterol efflux does not simply reflect the binding of HDL to cells, inasmuch as binding of HDL to CD36, which is another HDL binding scavenger receptor, does not facilitate cholesterol efflux.	bind
22746	6	6382	7	NULL	NULL	NULL	NULL	statement 5	Process		does not facilitate					cholesterol	Chemical	efflux of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_13_s_150	11145929	102  However, SR-BI - mediated cholesterol efflux does not simply reflect the binding of HDL to cells, inasmuch as binding of HDL to CD36, which is another HDL binding scavenger receptor, does not facilitate cholesterol efflux.	bind
19634	1	6383	5	NULL	NULL	0	NULL	HDL	NULL		bind	NULL				SR-BI	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_13_s_151	11145929	103  Therefore, it has been suggested that binding of HDL to SR-BI facilitates the bidirectional flux between HDL and plasma membrane by reorganization of lipids within cholesterol- and caveolae-rich domains within the plasma membrane.	bind
19635	2	6383	5	NULL	NULL	0	NULL	statement 1	NULL		facilitates	NULL				bidirectional flux	NULL				NULL	between HDL and plasma membrane	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_13_s_151	11145929	103  Therefore, it has been suggested that binding of HDL to SR-BI facilitates the bidirectional flux between HDL and plasma membrane by reorganization of lipids within cholesterol- and caveolae-rich domains within the plasma membrane.	bind
19636	3	6383	5	NULL	NULL	0	NULL	lipids	NULL		are reorganized within	NULL					NULL		cholesterol-rich domains		NULL	within the plasma membrane	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_13_s_151	11145929	103  Therefore, it has been suggested that binding of HDL to SR-BI facilitates the bidirectional flux between HDL and plasma membrane by reorganization of lipids within cholesterol- and caveolae-rich domains within the plasma membrane.	bind
19637	4	6383	5	NULL	NULL	0	NULL	lipids	NULL		are reorganized within	NULL					NULL		caveolae-rich domains		NULL	within the plasma membrane	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_13_s_151	11145929	103  Therefore, it has been suggested that binding of HDL to SR-BI facilitates the bidirectional flux between HDL and plasma membrane by reorganization of lipids within cholesterol- and caveolae-rich domains within the plasma membrane.	bind
19638	5	6383	5	NULL	NULL	0	NULL	statement 3	NULL		is required for	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_13_s_151	11145929	103  Therefore, it has been suggested that binding of HDL to SR-BI facilitates the bidirectional flux between HDL and plasma membrane by reorganization of lipids within cholesterol- and caveolae-rich domains within the plasma membrane.	bind
19639	6	6383	5	NULL	NULL	0	NULL	statement 4	NULL		is required for	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_13_s_151	11145929	103  Therefore, it has been suggested that binding of HDL to SR-BI facilitates the bidirectional flux between HDL and plasma membrane by reorganization of lipids within cholesterol- and caveolae-rich domains within the plasma membrane.	bind
22747	1	6383	7	NULL	NULL	NULL	NULL	HDL	GP		bind					SR-BI	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_13_s_151	11145929	103  Therefore, it has been suggested that binding of HDL to SR-BI facilitates the bidirectional flux between HDL and plasma membrane by reorganization of lipids within cholesterol- and caveolae-rich domains within the plasma membrane.	bind
22749	2	6383	7	NULL	NULL	NULL	NULL	statement 1	Process		facilitate					bidirectional flux	Process				NULL	between HDL and plasma membrane 	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_13_s_151	11145929	103  Therefore, it has been suggested that binding of HDL to SR-BI facilitates the bidirectional flux between HDL and plasma membrane by reorganization of lipids within cholesterol- and caveolae-rich domains within the plasma membrane.	bind
22752	3	6383	7	NULL	NULL	NULL	NULL	lipids	Chemical		are reorganized within								cholesterol-rich domains		NULL	within the plasma membrane	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_13_s_151	11145929	103  Therefore, it has been suggested that binding of HDL to SR-BI facilitates the bidirectional flux between HDL and plasma membrane by reorganization of lipids within cholesterol- and caveolae-rich domains within the plasma membrane.	bind
22753	4	6383	7	NULL	NULL	NULL	NULL	lipids	Chemical		are reorganized within								caveolae-rich domains 		NULL	within the plasma membrane	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_13_s_151	11145929	103  Therefore, it has been suggested that binding of HDL to SR-BI facilitates the bidirectional flux between HDL and plasma membrane by reorganization of lipids within cholesterol- and caveolae-rich domains within the plasma membrane.	bind
45660	5	6383	7	NULL	NULL	NULL	NULL	statement 3	Process		is required for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_13_s_151	11145929	103  Therefore, it has been suggested that binding of HDL to SR-BI facilitates the bidirectional flux between HDL and plasma membrane by reorganization of lipids within cholesterol- and caveolae-rich domains within the plasma membrane.	bind
45661	6	6383	7	NULL	NULL	NULL	NULL	statement 4	Process		is required for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_13_s_151	11145929	103  Therefore, it has been suggested that binding of HDL to SR-BI facilitates the bidirectional flux between HDL and plasma membrane by reorganization of lipids within cholesterol- and caveolae-rich domains within the plasma membrane.	bind
19640	1	6384	5	NULL	NULL	0	NULL	c-Jun	NULL		bind	NULL	enhanced				NULL			AP-1 - binding sites	NULL	kidneys	0	NULL	NULL	NULL	gw60_circulationres_79_2_162_s_311	8755992	104  Such kidneys also display enhanced binding of c-Jun and ATF2 (both substrates for JNK/SAPKs 22  23 43 44 ) to AP-1 - binding sites and cAMP response elements.	bind
19641	2	6384	5	NULL	NULL	0	NULL	c-Jun	NULL		bind	NULL	enhanced				NULL			cAMP response elements	NULL	kidneys	NULL	NULL	NULL	NULL	gw60_circulationres_79_2_162_s_311	8755992	104  Such kidneys also display enhanced binding of c-Jun and ATF2 (both substrates for JNK/SAPKs 22  23 43 44 ) to AP-1 - binding sites and cAMP response elements.	bind
19642	3	6384	5	10	NULL	0	NULL	ATF2			bind		enhanced							AP-1 - binding sites	NULL	kidneys	NULL	NULL	NULL	NULL	gw60_circulationres_79_2_162_s_311	8755992	104  Such kidneys also display enhanced binding of c-Jun and ATF2 (both substrates for JNK/SAPKs 22  23 43 44 ) to AP-1 - binding sites and cAMP response elements.	bind
19643	4	6384	5	10	NULL	0	NULL	ATF2			bind		enhanced							cAMP response elements	NULL	kidneys	NULL	NULL	NULL	NULL	gw60_circulationres_79_2_162_s_311	8755992	104  Such kidneys also display enhanced binding of c-Jun and ATF2 (both substrates for JNK/SAPKs 22  23 43 44 ) to AP-1 - binding sites and cAMP response elements.	bind
19644	5	6384	5	NULL	NULL	0	NULL	c-Jun	NULL		is a substrate for	NULL				JNK/SAPKs	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_79_2_162_s_311	8755992	104  Such kidneys also display enhanced binding of c-Jun and ATF2 (both substrates for JNK/SAPKs 22  23 43 44 ) to AP-1 - binding sites and cAMP response elements.	bind
19645	6	6384	5	NULL	NULL	0	NULL	ATF2	NULL		is a substrate for	NULL				JNK/SAPKs	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_79_2_162_s_311	8755992	104  Such kidneys also display enhanced binding of c-Jun and ATF2 (both substrates for JNK/SAPKs 22  23 43 44 ) to AP-1 - binding sites and cAMP response elements.	bind
22756	1	6384	7	NULL	NULL	NULL	NULL	c-Jun	GP		bind									AP-1 - binding sites	NULL	kidneys	NULL	NULL	NULL	NULL	gw60_circulationres_79_2_162_s_311	8755992	104  Such kidneys also display enhanced binding of c-Jun and ATF2 (both substrates for JNK/SAPKs 22  23 43 44 ) to AP-1 - binding sites and cAMP response elements.	bind
22757	2	6384	7	NULL	NULL	NULL	NULL	ATF2	GP		bind									cAMP response element	NULL	kidneys	NULL	NULL	NULL	NULL	gw60_circulationres_79_2_162_s_311	8755992	104  Such kidneys also display enhanced binding of c-Jun and ATF2 (both substrates for JNK/SAPKs 22  23 43 44 ) to AP-1 - binding sites and cAMP response elements.	bind
22758	3	6384	7	NULL	NULL	NULL	NULL	c-Jun 	GP		is a substrate for					JNK/SAPKs	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_2_162_s_311	8755992	104  Such kidneys also display enhanced binding of c-Jun and ATF2 (both substrates for JNK/SAPKs 22  23 43 44 ) to AP-1 - binding sites and cAMP response elements.	bind
22759	4	6384	7	NULL	NULL	NULL	NULL	ATF2	GP		is a substrate for					JNK/SAPKs	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_2_162_s_311	8755992	104  Such kidneys also display enhanced binding of c-Jun and ATF2 (both substrates for JNK/SAPKs 22  23 43 44 ) to AP-1 - binding sites and cAMP response elements.	bind
54248	5	6384	7	NULL	NULL	NULL	NULL	c-Jun	GP		bind									cAMP response elements	NULL	kidneys	NULL	NULL	NULL	NULL	gw60_circulationres_79_2_162_s_311	8755992	104  Such kidneys also display enhanced binding of c-Jun and ATF2 (both substrates for JNK/SAPKs 22  23 43 44 ) to AP-1 - binding sites and cAMP response elements.	bind
54249	6	6384	7	NULL	NULL	NULL	NULL	ATF2	GP		bind									AP-1 - binding sites	NULL	kidneys	NULL	NULL	NULL	NULL	gw60_circulationres_79_2_162_s_311	8755992	104  Such kidneys also display enhanced binding of c-Jun and ATF2 (both substrates for JNK/SAPKs 22  23 43 44 ) to AP-1 - binding sites and cAMP response elements.	bind
19646	1	6386	5	NULL	NULL	0	NULL	MTP	NULL		bind	NULL				apoB	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_887_s_139	11397693	108  It has been recently reported that an MTP inhibitor (AGI-S17) blocked MTP-apoB binding and the secretion of apoB without interfering with MTP lipid transfer activity.	bind
19647	2	6386	5	NULL	NULL	0	NULL	AGI-S17	NULL		is a type of	NULL				MTP inhibitor	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_887_s_139	11397693	108  It has been recently reported that an MTP inhibitor (AGI-S17) blocked MTP-apoB binding and the secretion of apoB without interfering with MTP lipid transfer activity.	bind
19648	3	6386	5	NULL	NULL	0	NULL	AGI-S17	NULL		blocks	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_887_s_139	11397693	108  It has been recently reported that an MTP inhibitor (AGI-S17) blocked MTP-apoB binding and the secretion of apoB without interfering with MTP lipid transfer activity.	bind
19649	4	6386	5	NULL	NULL	0	NULL	AGI-S17	NULL		blocks	NULL				apoB	NULL	secretion of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_887_s_139	11397693	108  It has been recently reported that an MTP inhibitor (AGI-S17) blocked MTP-apoB binding and the secretion of apoB without interfering with MTP lipid transfer activity.	bind
19650	6	6386	5	NULL	NULL	0	NULL	statement 4	NULL		does not interfere with	NULL				statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_887_s_139	11397693	108  It has been recently reported that an MTP inhibitor (AGI-S17) blocked MTP-apoB binding and the secretion of apoB without interfering with MTP lipid transfer activity.	bind
28696	7	6386	5	NULL	NULL	0	NULL	statement 3	NULL		does not interfere with	NULL				statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_887_s_139	11397693	108  It has been recently reported that an MTP inhibitor (AGI-S17) blocked MTP-apoB binding and the secretion of apoB without interfering with MTP lipid transfer activity.	bind
46203	5	6386	5	NULL	NULL	0	NULL	MTP	NULL		exhibits	NULL				lipid transfer activity	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_887_s_139	11397693	108  It has been recently reported that an MTP inhibitor (AGI-S17) blocked MTP-apoB binding and the secretion of apoB without interfering with MTP lipid transfer activity.	bind
22760	1	6386	7	NULL	NULL	NULL	NULL	MTP	GP		bind					apoB	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_887_s_139	11397693	108  It has been recently reported that an MTP inhibitor (AGI-S17) blocked MTP-apoB binding and the secretion of apoB without interfering with MTP lipid transfer activity.	bind
22761	2	6386	7	NULL	NULL	NULL	NULL	AGI-S17	Chemical		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_887_s_139	11397693	108  It has been recently reported that an MTP inhibitor (AGI-S17) blocked MTP-apoB binding and the secretion of apoB without interfering with MTP lipid transfer activity.	bind
22763	3	6386	7	NULL	NULL	NULL	NULL	AGI-S17	Chemical		blocks					apoB	Chemical	secretion of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_887_s_139	11397693	108  It has been recently reported that an MTP inhibitor (AGI-S17) blocked MTP-apoB binding and the secretion of apoB without interfering with MTP lipid transfer activity.	bind
22765	5	6386	7	NULL	NULL	NULL	NULL	statement 2	Process		does not interfere with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_887_s_139	11397693	108  It has been recently reported that an MTP inhibitor (AGI-S17) blocked MTP-apoB binding and the secretion of apoB without interfering with MTP lipid transfer activity.	bind
22766	6	6386	7	NULL	NULL	NULL	NULL	statement 3	Process		does not interfere with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_887_s_139	11397693	108  It has been recently reported that an MTP inhibitor (AGI-S17) blocked MTP-apoB binding and the secretion of apoB without interfering with MTP lipid transfer activity.	bind
29398	7	6386	7	NULL	NULL	NULL	NULL	AGI-S17	Chemical		is a type of					MTP inhibitor	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_887_s_139	11397693	108  It has been recently reported that an MTP inhibitor (AGI-S17) blocked MTP-apoB binding and the secretion of apoB without interfering with MTP lipid transfer activity.	bind
45662	4	6386	7	NULL	NULL	NULL	NULL	MTP	GP		exhibits					lipid transfer activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_887_s_139	11397693	108  It has been recently reported that an MTP inhibitor (AGI-S17) blocked MTP-apoB binding and the secretion of apoB without interfering with MTP lipid transfer activity.	bind
19651	1	6387	5	NULL	NULL	0	NULL	prothrombin	NULL		bind	NULL				GP IIb-IIIa	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_177	12231555	108 -  111 One group has suggested that prothrombin binding to GP IIb-IIIa may provide a pool of prothrombin for activation by the factor Xa/Va complex and that abciximab may decrease thrombin generation by blocking prothrombin binding.	bind
19652	2	6387	5	10	NULL	0	NULL	prothrombin			is activated by					factor Xa/Va complex					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_177	12231555	108 -  111 One group has suggested that prothrombin binding to GP IIb-IIIa may provide a pool of prothrombin for activation by the factor Xa/Va complex and that abciximab may decrease thrombin generation by blocking prothrombin binding.	bind
19653	3	6387	5	NULL	NULL	0	NULL	statement 1	NULL		lead to	NULL	may			statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_177	12231555	108 -  111 One group has suggested that prothrombin binding to GP IIb-IIIa may provide a pool of prothrombin for activation by the factor Xa/Va complex and that abciximab may decrease thrombin generation by blocking prothrombin binding.	bind
19654	4	6387	5	NULL	NULL	0	NULL	abciximab	NULL		blocks	NULL				prothrombin	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_177	12231555	108 -  111 One group has suggested that prothrombin binding to GP IIb-IIIa may provide a pool of prothrombin for activation by the factor Xa/Va complex and that abciximab may decrease thrombin generation by blocking prothrombin binding.	bind
19655	5	6387	5	NULL	NULL	0	NULL	abciximab	NULL		decrease	NULL	may			thrombin	NULL	generation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_177	12231555	108 -  111 One group has suggested that prothrombin binding to GP IIb-IIIa may provide a pool of prothrombin for activation by the factor Xa/Va complex and that abciximab may decrease thrombin generation by blocking prothrombin binding.	bind
19656	6	6387	5	NULL	NULL	0	NULL	statement 4	NULL		leads to	NULL				statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_177	12231555	108 -  111 One group has suggested that prothrombin binding to GP IIb-IIIa may provide a pool of prothrombin for activation by the factor Xa/Va complex and that abciximab may decrease thrombin generation by blocking prothrombin binding.	bind
22767	1	6387	7	NULL	NULL	NULL	NULL	prothrombin	GP		bind					GP IIb-IIIa	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_177	12231555	108 -  111 One group has suggested that prothrombin binding to GP IIb-IIIa may provide a pool of prothrombin for activation by the factor Xa/Va complex and that abciximab may decrease thrombin generation by blocking prothrombin binding.	bind
22768	2	6387	7	NULL	NULL	NULL	NULL	factor Xa/Va complex	GP		activate					prothrombin	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_177	12231555	108 -  111 One group has suggested that prothrombin binding to GP IIb-IIIa may provide a pool of prothrombin for activation by the factor Xa/Va complex and that abciximab may decrease thrombin generation by blocking prothrombin binding.	bind
22769	3	6387	7	NULL	NULL	NULL	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_177	12231555	108 -  111 One group has suggested that prothrombin binding to GP IIb-IIIa may provide a pool of prothrombin for activation by the factor Xa/Va complex and that abciximab may decrease thrombin generation by blocking prothrombin binding.	bind
22770	4	6387	7	NULL	NULL	NULL	NULL	abciximab	Chemical		blocks					prothrombin	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_177	12231555	108 -  111 One group has suggested that prothrombin binding to GP IIb-IIIa may provide a pool of prothrombin for activation by the factor Xa/Va complex and that abciximab may decrease thrombin generation by blocking prothrombin binding.	bind
22771	5	6387	7	NULL	NULL	NULL	NULL	abciximab	Chemical		decrease		may			thrombin	GP	generation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_177	12231555	108 -  111 One group has suggested that prothrombin binding to GP IIb-IIIa may provide a pool of prothrombin for activation by the factor Xa/Va complex and that abciximab may decrease thrombin generation by blocking prothrombin binding.	bind
22772	6	6387	7	NULL	NULL	NULL	NULL	statement 5	Process		occurs by					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_177	12231555	108 -  111 One group has suggested that prothrombin binding to GP IIb-IIIa may provide a pool of prothrombin for activation by the factor Xa/Va complex and that abciximab may decrease thrombin generation by blocking prothrombin binding.	bind
19657	1	6388	5	NULL	NULL	0	NULL	ferritin	NULL		bind	NULL					NULL		VL-domain		NULL		0	NULL	NULL	NULL	abs-batch0650-0679_biochemistry-(mosc)_65_9_11042491_s_9	11042491	108 M(-1)) is similar to the affinity of  the full-length parental antibody F11 because when the immobilized VL-domain  was used, the binding constant of ferritin to the VL-domain was only 4-6-fold  lower than that in the case of F11 antibody.	bind
22773	1	6388	7	NULL	NULL	NULL	NULL	ferritin	GP		bind								VL-domain		NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochemistry-(mosc)_65_9_11042491_s_9	11042491	108 M(-1)) is similar to the affinity of  the full-length parental antibody F11 because when the immobilized VL-domain  was used, the binding constant of ferritin to the VL-domain was only 4-6-fold  lower than that in the case of F11 antibody.	bind
19658	1	6390	5	NULL	NULL	0	NULL	transcription factor	NULL		bind	NULL				HER2	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_21_4257_s_210	11691913	11       Noonberg,S.B., Scott,G.K., Hunt,C.A., Hogan,M.E. and Benz,C.C. (1994) Inhibition of transcription factor binding to the HER2 promoter by triplex-forming oligodeoxyribonucleotides.	bind
19659	2	6390	5	NULL	NULL	0	NULL	oligodeoxyribonucleotides	NULL	triplex-forming	inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_21_4257_s_210	11691913	11       Noonberg,S.B., Scott,G.K., Hunt,C.A., Hogan,M.E. and Benz,C.C. (1994) Inhibition of transcription factor binding to the HER2 promoter by triplex-forming oligodeoxyribonucleotides.	bind
22775	1	6390	7	NULL	NULL	NULL	NULL	transcription factor	GP		bind					HER2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_21_4257_s_210	11691913	11       Noonberg,S.B., Scott,G.K., Hunt,C.A., Hogan,M.E. and Benz,C.C. (1994) Inhibition of transcription factor binding to the HER2 promoter by triplex-forming oligodeoxyribonucleotides.	bind
22776	2	6390	7	NULL	NULL	NULL	NULL	oligodeoxyribonucleotides	NucleicAcid	triplex-forming	inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_21_4257_s_210	11691913	11       Noonberg,S.B., Scott,G.K., Hunt,C.A., Hogan,M.E. and Benz,C.C. (1994) Inhibition of transcription factor binding to the HER2 promoter by triplex-forming oligodeoxyribonucleotides.	bind
19660	1	6391	5	NULL	NULL	0	NULL	DpnM DNA adenine methyltransferase	NULL	DpnII restriction system of Streptococcus pneumoniae	bind	NULL				S-adenosylmethionine	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_15_3137_s_242	11470870	11       Tran,P.H., Korszun,Z.R., Cerritelli,S., Springhorn,S.S. and Lacks,S.A. (1998) Crystal structure of the  DpnM DNA adenine methyltransferase from the  DpnII restriction system of  Streptococcus pneumoniae bound to S-adenosylmethionine.	bind
22777	1	6391	7	NULL	NULL	NULL	NULL	DpnM DNA adenine methyltransferase	GP	streptococcus pneumoniae	bind					S-adenosylmethionine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_15_3137_s_242	11470870	11       Tran,P.H., Korszun,Z.R., Cerritelli,S., Springhorn,S.S. and Lacks,S.A. (1998) Crystal structure of the  DpnM DNA adenine methyltransferase from the  DpnII restriction system of  Streptococcus pneumoniae bound to S-adenosylmethionine.	bind
22778	2	6391	7	NULL	NULL	NULL	NULL	DpnM DNA adenine methyltransferase	GP		is derived from					DpnII restriction system	GP	Streptococcus pneumoniae			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_15_3137_s_242	11470870	11       Tran,P.H., Korszun,Z.R., Cerritelli,S., Springhorn,S.S. and Lacks,S.A. (1998) Crystal structure of the  DpnM DNA adenine methyltransferase from the  DpnII restriction system of  Streptococcus pneumoniae bound to S-adenosylmethionine.	bind
19661	1	6392	5	NULL	NULL	0	NULL	MDM2 protein	NULL		interacts with	NULL	specifically	central acidic domain		L5 protein	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_2_587_s_21	10934161	11  A possible function of MDM2 protein in ribosome biosynthesis or in translational regulation is suggested by the specific interaction of the central acidic domain of the MDM2 protein with the L5 protein, a component of a large ribosomal subunit, which is itself associated with 5s rRNA. 12, 13  A positive correlation was found between MDM2 binding to TAFII250 and activation of cyclin A, a regulator of the cell cycle.	bind
19662	2	6392	5	10	NULL	0	NULL	L5 protein			is a component of					large ribosomal subunit					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_587_s_21	10934161	11  A possible function of MDM2 protein in ribosome biosynthesis or in translational regulation is suggested by the specific interaction of the central acidic domain of the MDM2 protein with the L5 protein, a component of a large ribosomal subunit, which is itself associated with 5s rRNA. 12, 13  A positive correlation was found between MDM2 binding to TAFII250 and activation of cyclin A, a regulator of the cell cycle.	bind
19663	3	6392	5	NULL	NULL	0	NULL	L5 protein	NULL		is associated with	NULL				5s rRNA	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_2_587_s_21	10934161	11  A possible function of MDM2 protein in ribosome biosynthesis or in translational regulation is suggested by the specific interaction of the central acidic domain of the MDM2 protein with the L5 protein, a component of a large ribosomal subunit, which is itself associated with 5s rRNA. 12, 13  A positive correlation was found between MDM2 binding to TAFII250 and activation of cyclin A, a regulator of the cell cycle.	bind
19664	4	6392	5	NULL	NULL	0	NULL	MDM2	NULL		bind	NULL				TAFII250	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_2_587_s_21	10934161	11  A possible function of MDM2 protein in ribosome biosynthesis or in translational regulation is suggested by the specific interaction of the central acidic domain of the MDM2 protein with the L5 protein, a component of a large ribosomal subunit, which is itself associated with 5s rRNA. 12, 13  A positive correlation was found between MDM2 binding to TAFII250 and activation of cyclin A, a regulator of the cell cycle.	bind
19665	5	6392	5	NULL	NULL	0	NULL	statement 4	NULL		correlates with	NULL	positively			cyclin A	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_2_587_s_21	10934161	11  A possible function of MDM2 protein in ribosome biosynthesis or in translational regulation is suggested by the specific interaction of the central acidic domain of the MDM2 protein with the L5 protein, a component of a large ribosomal subunit, which is itself associated with 5s rRNA. 12, 13  A positive correlation was found between MDM2 binding to TAFII250 and activation of cyclin A, a regulator of the cell cycle.	bind
19666	6	6392	5	NULL	NULL	0	NULL	cyclin A	NULL		is	NULL				a regulator of cell cycle	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_2_587_s_21	10934161	11  A possible function of MDM2 protein in ribosome biosynthesis or in translational regulation is suggested by the specific interaction of the central acidic domain of the MDM2 protein with the L5 protein, a component of a large ribosomal subunit, which is itself associated with 5s rRNA. 12, 13  A positive correlation was found between MDM2 binding to TAFII250 and activation of cyclin A, a regulator of the cell cycle.	bind
54250	7	6392	5	10	NULL	0	NULL	MDM2 protein			function in		possibly			ribosome		biosynthesis of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_2_587_s_21	10934161	11  A possible function of MDM2 protein in ribosome biosynthesis or in translational regulation is suggested by the specific interaction of the central acidic domain of the MDM2 protein with the L5 protein, a component of a large ribosomal subunit, which is itself associated with 5s rRNA. 12, 13  A positive correlation was found between MDM2 binding to TAFII250 and activation of cyclin A, a regulator of the cell cycle.	bind
54251	8	6392	5	10	NULL	0	NULL	MDM2 protein			function in		possibly			translation		regulation of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_2_587_s_21	10934161	11  A possible function of MDM2 protein in ribosome biosynthesis or in translational regulation is suggested by the specific interaction of the central acidic domain of the MDM2 protein with the L5 protein, a component of a large ribosomal subunit, which is itself associated with 5s rRNA. 12, 13  A positive correlation was found between MDM2 binding to TAFII250 and activation of cyclin A, a regulator of the cell cycle.	bind
54252	9	6392	5	10	NULL	0	NULL	statement 1			suggests					statement 7					NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_2_587_s_21	10934161	11  A possible function of MDM2 protein in ribosome biosynthesis or in translational regulation is suggested by the specific interaction of the central acidic domain of the MDM2 protein with the L5 protein, a component of a large ribosomal subunit, which is itself associated with 5s rRNA. 12, 13  A positive correlation was found between MDM2 binding to TAFII250 and activation of cyclin A, a regulator of the cell cycle.	bind
54253	10	6392	5	10	NULL	0	NULL	statement 1			suggests					statement 8					NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_2_587_s_21	10934161	11  A possible function of MDM2 protein in ribosome biosynthesis or in translational regulation is suggested by the specific interaction of the central acidic domain of the MDM2 protein with the L5 protein, a component of a large ribosomal subunit, which is itself associated with 5s rRNA. 12, 13  A positive correlation was found between MDM2 binding to TAFII250 and activation of cyclin A, a regulator of the cell cycle.	bind
22779	1	6392	7	NULL	NULL	NULL	NULL	MDM2 protein	GP		interacts with		specifically	central acidic domain 		L5 protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_587_s_21	10934161	11  A possible function of MDM2 protein in ribosome biosynthesis or in translational regulation is suggested by the specific interaction of the central acidic domain of the MDM2 protein with the L5 protein, a component of a large ribosomal subunit, which is itself associated with 5s rRNA. 12, 13  A positive correlation was found between MDM2 binding to TAFII250 and activation of cyclin A, a regulator of the cell cycle.	bind
22780	2	6392	7	NULL	NULL	NULL	NULL	statement 1	Process		suggests					statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_587_s_21	10934161	11  A possible function of MDM2 protein in ribosome biosynthesis or in translational regulation is suggested by the specific interaction of the central acidic domain of the MDM2 protein with the L5 protein, a component of a large ribosomal subunit, which is itself associated with 5s rRNA. 12, 13  A positive correlation was found between MDM2 binding to TAFII250 and activation of cyclin A, a regulator of the cell cycle.	bind
22781	3	6392	7	NULL	NULL	NULL	NULL	statement 1	Process		suggests					statement 10	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_587_s_21	10934161	11  A possible function of MDM2 protein in ribosome biosynthesis or in translational regulation is suggested by the specific interaction of the central acidic domain of the MDM2 protein with the L5 protein, a component of a large ribosomal subunit, which is itself associated with 5s rRNA. 12, 13  A positive correlation was found between MDM2 binding to TAFII250 and activation of cyclin A, a regulator of the cell cycle.	bind
22783	4	6392	7	NULL	NULL	NULL	NULL	L5 protein	GP		is a component of					large ribosomal subunit	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_587_s_21	10934161	11  A possible function of MDM2 protein in ribosome biosynthesis or in translational regulation is suggested by the specific interaction of the central acidic domain of the MDM2 protein with the L5 protein, a component of a large ribosomal subunit, which is itself associated with 5s rRNA. 12, 13  A positive correlation was found between MDM2 binding to TAFII250 and activation of cyclin A, a regulator of the cell cycle.	bind
22784	5	6392	7	NULL	NULL	NULL	NULL	L5 protein	GP		associate with					5s rRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_587_s_21	10934161	11  A possible function of MDM2 protein in ribosome biosynthesis or in translational regulation is suggested by the specific interaction of the central acidic domain of the MDM2 protein with the L5 protein, a component of a large ribosomal subunit, which is itself associated with 5s rRNA. 12, 13  A positive correlation was found between MDM2 binding to TAFII250 and activation of cyclin A, a regulator of the cell cycle.	bind
22787	6	6392	7	NULL	NULL	NULL	NULL	MDM2	GP		bind					TAFII250	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_587_s_21	10934161	11  A possible function of MDM2 protein in ribosome biosynthesis or in translational regulation is suggested by the specific interaction of the central acidic domain of the MDM2 protein with the L5 protein, a component of a large ribosomal subunit, which is itself associated with 5s rRNA. 12, 13  A positive correlation was found between MDM2 binding to TAFII250 and activation of cyclin A, a regulator of the cell cycle.	bind
22795	7	6392	7	NULL	NULL	NULL	NULL	cyclin A	GP	activation of	regulates					cell cycle	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_587_s_21	10934161	11  A possible function of MDM2 protein in ribosome biosynthesis or in translational regulation is suggested by the specific interaction of the central acidic domain of the MDM2 protein with the L5 protein, a component of a large ribosomal subunit, which is itself associated with 5s rRNA. 12, 13  A positive correlation was found between MDM2 binding to TAFII250 and activation of cyclin A, a regulator of the cell cycle.	bind
22797	8	6392	7	NULL	NULL	NULL	NULL	statement 6	Process		correlates with		positively			statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_587_s_21	10934161	11  A possible function of MDM2 protein in ribosome biosynthesis or in translational regulation is suggested by the specific interaction of the central acidic domain of the MDM2 protein with the L5 protein, a component of a large ribosomal subunit, which is itself associated with 5s rRNA. 12, 13  A positive correlation was found between MDM2 binding to TAFII250 and activation of cyclin A, a regulator of the cell cycle.	bind
54254	9	6392	7	NULL	NULL	NULL	NULL	MDM2 protein	GP		function in		possibly			ribosome	CellComponent	biosynthesis of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_587_s_21	10934161	11  A possible function of MDM2 protein in ribosome biosynthesis or in translational regulation is suggested by the specific interaction of the central acidic domain of the MDM2 protein with the L5 protein, a component of a large ribosomal subunit, which is itself associated with 5s rRNA. 12, 13  A positive correlation was found between MDM2 binding to TAFII250 and activation of cyclin A, a regulator of the cell cycle.	bind
54255	10	6392	7	NULL	NULL	NULL	NULL	MDM2 protein	GP		function in		possibly			translation	Process	regulation of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_587_s_21	10934161	11  A possible function of MDM2 protein in ribosome biosynthesis or in translational regulation is suggested by the specific interaction of the central acidic domain of the MDM2 protein with the L5 protein, a component of a large ribosomal subunit, which is itself associated with 5s rRNA. 12, 13  A positive correlation was found between MDM2 binding to TAFII250 and activation of cyclin A, a regulator of the cell cycle.	bind
19751	1	6393	5	10	NULL	0	NULL	cdc25A	NULL	ectopic expression of 	results in	NULL				cdc25A	NULL	higher levels of expression of 			NULL	VSM-myc cells	NULL	NULL	NULL	NULL	gw60_circulationres_84_7_820_s_126	10205150	11  Ectopic expression of cdc25A resulted in higher levels of cdc25A expression in all clones of VSM-myc cells irrespective of their c-Myc expression.	bind
45618	2	6393	5	10	NULL	0	NULL	statement 1	NULL		is irrespective of	NULL				c-Myc	NULL	expression of			NULL		0	NULL	NULL	NULL	gw60_circulationres_84_7_820_s_126	10205150	11  Ectopic expression of cdc25A resulted in higher levels of cdc25A expression in all clones of VSM-myc cells irrespective of their c-Myc expression.	bind
22828	1	6393	7	NULL	NULL	NULL	NULL	cdc25A	GP	Ectopic expression of	results in					cdc25A	GP	higher expression of			NULL	VSM-myc cells	NULL	NULL	NULL	NULL	gw60_circulationres_84_7_820_s_126	10205150	11  Ectopic expression of cdc25A resulted in higher levels of cdc25A expression in all clones of VSM-myc cells irrespective of their c-Myc expression.	bind
22829	2	6393	7	NULL	NULL	NULL	NULL	statement 1	Process		is irrespective of					c-Myc	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_7_820_s_126	10205150	11  Ectopic expression of cdc25A resulted in higher levels of cdc25A expression in all clones of VSM-myc cells irrespective of their c-Myc expression.	bind
19752	1	6394	5	NULL	NULL	0	NULL	apo E	NULL		plays a role in	NULL	important			TG-rich lipoproteins	NULL	catabolism of 			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_963_s_29	7600129	11  Even if all studies suggest an important role for apo E in the catabolism of TG-rich lipoproteins and an inhibitory effect of lipids and C apolipoproteins for apo B binding to the LDL receptor, no one can definitively determine the individual effect of each factor.	bind
19753	2	6394	5	NULL	NULL	0	NULL	apo B	NULL		bind	NULL				LDL receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_963_s_29	7600129	11  Even if all studies suggest an important role for apo E in the catabolism of TG-rich lipoproteins and an inhibitory effect of lipids and C apolipoproteins for apo B binding to the LDL receptor, no one can definitively determine the individual effect of each factor.	bind
19754	3	6394	5	NULL	NULL	0	NULL	lipids	NULL		inhibit	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_963_s_29	7600129	11  Even if all studies suggest an important role for apo E in the catabolism of TG-rich lipoproteins and an inhibitory effect of lipids and C apolipoproteins for apo B binding to the LDL receptor, no one can definitively determine the individual effect of each factor.	bind
19755	4	6394	5	NULL	NULL	0	NULL	C apolipoproteins	NULL		inhibit	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_963_s_29	7600129	11  Even if all studies suggest an important role for apo E in the catabolism of TG-rich lipoproteins and an inhibitory effect of lipids and C apolipoproteins for apo B binding to the LDL receptor, no one can definitively determine the individual effect of each factor.	bind
22830	1	6394	7	NULL	NULL	NULL	NULL	apo E	GP		plays a role in		importantly			 TG-rich lipoproteins	GP	catabolism of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_963_s_29	7600129	11  Even if all studies suggest an important role for apo E in the catabolism of TG-rich lipoproteins and an inhibitory effect of lipids and C apolipoproteins for apo B binding to the LDL receptor, no one can definitively determine the individual effect of each factor.	bind
22831	2	6394	7	NULL	NULL	NULL	NULL	apo B	GP		bind					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_963_s_29	7600129	11  Even if all studies suggest an important role for apo E in the catabolism of TG-rich lipoproteins and an inhibitory effect of lipids and C apolipoproteins for apo B binding to the LDL receptor, no one can definitively determine the individual effect of each factor.	bind
22832	3	6394	7	NULL	NULL	NULL	NULL	lipids	Chemical		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_963_s_29	7600129	11  Even if all studies suggest an important role for apo E in the catabolism of TG-rich lipoproteins and an inhibitory effect of lipids and C apolipoproteins for apo B binding to the LDL receptor, no one can definitively determine the individual effect of each factor.	bind
22833	4	6394	7	NULL	NULL	NULL	NULL	C apolipoproteins	GP		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_963_s_29	7600129	11  Even if all studies suggest an important role for apo E in the catabolism of TG-rich lipoproteins and an inhibitory effect of lipids and C apolipoproteins for apo B binding to the LDL receptor, no one can definitively determine the individual effect of each factor.	bind
19756	1	6395	5	10	NULL	0	NULL	Sp1	NULL	porcine;; endothelial cells	bind	NULL				TF	NULL			oligonucleotide spanning two putative Sp1 sites in promoter	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_2_365_s_261	9081693	11  Furthermore, Sp1 from porcine endothelial cells bound to an oligonucleotide spanning two putative Sp1 sites in the porcine TF promoter, 11  one of which is equivalent to Sp1V.	bind
19757	2	6395	5	10	NULL	0	NULL	TF	NULL	porcine	is equivalent to	NULL			putative Sp1 site in promoter		NULL			Sp1V	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_2_365_s_261	9081693	11  Furthermore, Sp1 from porcine endothelial cells bound to an oligonucleotide spanning two putative Sp1 sites in the porcine TF promoter, 11  one of which is equivalent to Sp1V.	bind
22834	1	6395	7	NULL	NULL	NULL	NULL	Sp1	GP	porcine;; endothelial cells	bind					TF	GP	porcine		oligonucleotide spanning two putative Sp1 sites in the promoter	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_2_365_s_261	9081693	11  Furthermore, Sp1 from porcine endothelial cells bound to an oligonucleotide spanning two putative Sp1 sites in the porcine TF promoter, 11  one of which is equivalent to Sp1V.	bind
22836	2	6395	7	NULL	NULL	NULL	NULL	TF	GP	porcine	is equivalent to				putative Sp1 site in the promoter					Sp1V	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_2_365_s_261	9081693	11  Furthermore, Sp1 from porcine endothelial cells bound to an oligonucleotide spanning two putative Sp1 sites in the porcine TF promoter, 11  one of which is equivalent to Sp1V.	bind
19777	1	6397	5	NULL	NULL	0	NULL	VLDLR sequence	NULL	human	is similar to	NULL				vitellogenin receptor	NULL	chicken			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_3_407_s_32	8630667	11  In addition, the human VLDLR shares 84% of its sequence with the chicken vitellogenin receptor, 12  which also binds VLDL and is required for the delivery of nutrients to the developing avian oocyte.	bind
19778	2	6397	5	NULL	NULL	0	NULL	VLDLR	NULL	human	bind	NULL				VLDL	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_3_407_s_32	8630667	11  In addition, the human VLDLR shares 84% of its sequence with the chicken vitellogenin receptor, 12  which also binds VLDL and is required for the delivery of nutrients to the developing avian oocyte.	bind
19779	3	6397	5	NULL	NULL	0	NULL	VLDLR	NULL		is required for	NULL				nutrients	NULL	delivery of			NULL	to the developing avian oocyte	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_3_407_s_32	8630667	11  In addition, the human VLDLR shares 84% of its sequence with the chicken vitellogenin receptor, 12  which also binds VLDL and is required for the delivery of nutrients to the developing avian oocyte.	bind
22839	1	6397	7	NULL	NULL	NULL	NULL	VLDLR	GP	human	binds					VLDL	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_3_407_s_32	8630667	11  In addition, the human VLDLR shares 84% of its sequence with the chicken vitellogenin receptor, 12  which also binds VLDL and is required for the delivery of nutrients to the developing avian oocyte.	bind
22840	2	6397	7	NULL	NULL	NULL	NULL	statement 1	Process		is required for					nutrients	Chemical	delivery of 			NULL	developing avian oocyte	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_3_407_s_32	8630667	11  In addition, the human VLDLR shares 84% of its sequence with the chicken vitellogenin receptor, 12  which also binds VLDL and is required for the delivery of nutrients to the developing avian oocyte.	bind
29401	3	6397	7	NULL	NULL	NULL	NULL	VLDLR 	GP	human	is similar to					vitellogenin receptor	GP	chicken			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_3_407_s_32	8630667	11  In addition, the human VLDLR shares 84% of its sequence with the chicken vitellogenin receptor, 12  which also binds VLDL and is required for the delivery of nutrients to the developing avian oocyte.	bind
19798	1	6398	5	NULL	NULL	0	NULL	apo B	NULL		bind	NULL				LDL receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_963_s_158	7600129	11  LpB was radiolabeled, enriched with lipids, and then incubated with apolipoproteins CI, CII, CIII, and E. Preliminary studies indicated that free apolipoproteins did not interfere with apo B binding to the LDL receptor (V. Clavey, PR, et al, unpublished data, 1994), so we did not remove free apolipoproteins.	bind
19803	2	6398	5	NULL	NULL	0	NULL	apolipoproteins	NULL	free	does not interfere with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_963_s_158	7600129	11  LpB was radiolabeled, enriched with lipids, and then incubated with apolipoproteins CI, CII, CIII, and E. Preliminary studies indicated that free apolipoproteins did not interfere with apo B binding to the LDL receptor (V. Clavey, PR, et al, unpublished data, 1994), so we did not remove free apolipoproteins.	bind
22841	1	6398	7	NULL	NULL	NULL	NULL	apo B 	GP		bind					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_963_s_158	7600129	11  LpB was radiolabeled, enriched with lipids, and then incubated with apolipoproteins CI, CII, CIII, and E. Preliminary studies indicated that free apolipoproteins did not interfere with apo B binding to the LDL receptor (V. Clavey, PR, et al, unpublished data, 1994), so we did not remove free apolipoproteins.	bind
22842	2	6398	7	NULL	NULL	NULL	NULL	apolipoproteins 	GP	free 	does not interfere with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_963_s_158	7600129	11  LpB was radiolabeled, enriched with lipids, and then incubated with apolipoproteins CI, CII, CIII, and E. Preliminary studies indicated that free apolipoproteins did not interfere with apo B binding to the LDL receptor (V. Clavey, PR, et al, unpublished data, 1994), so we did not remove free apolipoproteins.	bind
19781	1	6399	5	NULL	NULL	0	NULL	caldesmon	NULL		bind	NULL				actin	NULL		low-affinity sites		NULL		0	NULL	NULL	NULL	gw60_circulationres_83_6_661_s_25	9742062	11  Numerous studies using in vitro reconstituted tropomyosin/actin/myosin complexes have shown that caldesmon binds actin at low- and high-affinity sites and that occupancy of the high-affinity site of actin is associated with a significant inhibition of actin-activated myosin ATPase activity.	bind
19782	2	6399	5	NULL	NULL	0	NULL	caldesmon	NULL		bind	NULL				actin	NULL		high-affinity sites		NULL		0	NULL	NULL	NULL	gw60_circulationres_83_6_661_s_25	9742062	11  Numerous studies using in vitro reconstituted tropomyosin/actin/myosin complexes have shown that caldesmon binds actin at low- and high-affinity sites and that occupancy of the high-affinity site of actin is associated with a significant inhibition of actin-activated myosin ATPase activity.	bind
19783	3	6399	5	10	NULL	0	NULL	actin	NULL		activates	NULL				myosin ATPase 	NULL	activity of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_6_661_s_25	9742062	11  Numerous studies using in vitro reconstituted tropomyosin/actin/myosin complexes have shown that caldesmon binds actin at low- and high-affinity sites and that occupancy of the high-affinity site of actin is associated with a significant inhibition of actin-activated myosin ATPase activity.	bind
19784	4	6399	5	NULL	NULL	0	NULL	actin	NULL	occupancy of	is associated with	NULL		high-affinity site		statement 3	NULL	significant inhibition of 			NULL		0	NULL	NULL	NULL	gw60_circulationres_83_6_661_s_25	9742062	11  Numerous studies using in vitro reconstituted tropomyosin/actin/myosin complexes have shown that caldesmon binds actin at low- and high-affinity sites and that occupancy of the high-affinity site of actin is associated with a significant inhibition of actin-activated myosin ATPase activity.	bind
22844	1	6399	7	NULL	NULL	NULL	NULL	caldesmon	GP		binds					actin	GP		low-affinity site		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_6_661_s_25	9742062	11  Numerous studies using in vitro reconstituted tropomyosin/actin/myosin complexes have shown that caldesmon binds actin at low- and high-affinity sites and that occupancy of the high-affinity site of actin is associated with a significant inhibition of actin-activated myosin ATPase activity.	bind
22845	2	6399	7	NULL	NULL	NULL	NULL	caldesmon	GP		binds					actin	GP		high-affinity site		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_6_661_s_25	9742062	11  Numerous studies using in vitro reconstituted tropomyosin/actin/myosin complexes have shown that caldesmon binds actin at low- and high-affinity sites and that occupancy of the high-affinity site of actin is associated with a significant inhibition of actin-activated myosin ATPase activity.	bind
22846	3	6399	7	NULL	NULL	NULL	NULL	actin	GP		activates					myosin ATPase 	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_6_661_s_25	9742062	11  Numerous studies using in vitro reconstituted tropomyosin/actin/myosin complexes have shown that caldesmon binds actin at low- and high-affinity sites and that occupancy of the high-affinity site of actin is associated with a significant inhibition of actin-activated myosin ATPase activity.	bind
22847	4	6399	7	NULL	NULL	NULL	NULL	actin	GP	occupancy	associate with			high-affinity site		statement 3	Process	inhibition of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_6_661_s_25	9742062	11  Numerous studies using in vitro reconstituted tropomyosin/actin/myosin complexes have shown that caldesmon binds actin at low- and high-affinity sites and that occupancy of the high-affinity site of actin is associated with a significant inhibition of actin-activated myosin ATPase activity.	bind
19780	1	6400	5	10	NULL	0	NULL	GAGs	NULL	highly sulfated	bind	NULL	high affinity			PDGF A isoform	NULL	long			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2897_s_214	9409273	11  Particularly highly sulfated GAGs bind the long PDGF A isoform with high affinity.	bind
22843	1	6400	7	NULL	NULL	NULL	NULL	GAGs	Chemical	highly sulfated	bind		high affinity			PDGF A isoform	GP	long			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2897_s_214	9409273	11  Particularly highly sulfated GAGs bind the long PDGF A isoform with high affinity.	bind
19804	1	6401	5	NULL	NULL	0	NULL	vWF	NULL		is	NULL				von Willebrand factor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_102_17_2045_s_24	11044418	11  Shear stress induces the binding of von Willebrand factor (vWF) to the GP Ib/IXV complex on platelets.	bind
19805	2	6401	5	NULL	NULL	0	NULL	vWF	NULL		bind	NULL				GP Ib/IXV complex	NULL				NULL	on platelets	0	NULL	NULL	NULL	gw60_circulation_102_17_2045_s_24	11044418	11  Shear stress induces the binding of von Willebrand factor (vWF) to the GP Ib/IXV complex on platelets.	bind
19928	3	6401	5	NULL	NULL	0	NULL	shear stress	NULL		induces	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_102_17_2045_s_24	11044418	11  Shear stress induces the binding of von Willebrand factor (vWF) to the GP Ib/IXV complex on platelets.	bind
22982	1	6401	7	NULL	NULL	NULL	NULL	vWF	GP		bind					GP Ib/IXV complex	GP				NULL	platelets	NULL	NULL	NULL	NULL	gw60_circulation_102_17_2045_s_24	11044418	11  Shear stress induces the binding of von Willebrand factor (vWF) to the GP Ib/IXV complex on platelets.	bind
22983	2	6401	7	NULL	NULL	NULL	NULL	shear stress	Process		induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_17_2045_s_24	11044418	11  Shear stress induces the binding of von Willebrand factor (vWF) to the GP Ib/IXV complex on platelets.	bind
22984	3	6401	7	NULL	NULL	NULL	NULL	vWF	GP		is					von Willebrand factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_17_2045_s_24	11044418	11  Shear stress induces the binding of von Willebrand factor (vWF) to the GP Ib/IXV complex on platelets.	bind
19929	1	6402	5	NULL	NULL	0	NULL	fibrinogen	NULL		bind	NULL				GPIIb/IIIa receptors	NULL	functional			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_12_2195_s_18	7489242	11  The binding of fibrinogen by functional GPIIb/IIIa receptors represents the final common step in platelet activation by all agonists.	bind
19930	2	6402	5	NULL	NULL	0	NULL	agonists	NULL		activates	NULL				platelets	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_12_2195_s_18	7489242	11  The binding of fibrinogen by functional GPIIb/IIIa receptors represents the final common step in platelet activation by all agonists.	bind
19931	3	6402	5	NULL	NULL	0	NULL	statement 1	NULL		is final step in	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_12_2195_s_18	7489242	11  The binding of fibrinogen by functional GPIIb/IIIa receptors represents the final common step in platelet activation by all agonists.	bind
22991	1	6402	7	NULL	NULL	NULL	NULL	fibrinogen	GP		bind					GPIIb/IIIa receptors	GP	functional			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_12_2195_s_18	7489242	11  The binding of fibrinogen by functional GPIIb/IIIa receptors represents the final common step in platelet activation by all agonists.	bind
22992	2	6402	7	NULL	NULL	NULL	NULL	agonists	Chemical		activates					platelet	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_12_2195_s_18	7489242	11  The binding of fibrinogen by functional GPIIb/IIIa receptors represents the final common step in platelet activation by all agonists.	bind
22993	3	6402	7	NULL	NULL	NULL	NULL	statement 1	Process		is final step in					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_12_2195_s_18	7489242	11  The binding of fibrinogen by functional GPIIb/IIIa receptors represents the final common step in platelet activation by all agonists.	bind
19933	1	6404	5	NULL	NULL	0	NULL	cell surface receptor	NULL		is linked to	NULL		transmembrane domain		tyrosine kinase	NULL	intracellular			NULL		NULL	NULL	NULL	NULL	gw60_circulation_94_8_1927_s_20	8873670	11  The molecule has a cell surface receptor linked by a transmembrane domain to an intracellular tyrosine kinase; it binds to heparin, basement membrane, and heparan sulfate components of the extracellular matrix, providing a tissue depot of bFGF.	bind
22996	1	6404	7	NULL	NULL	NULL	NULL	cell surface receptor	GP		is linked to			transmembrane domain		tyrosine kinase	GP	intracellular			NULL		NULL	NULL	NULL	NULL	gw60_circulation_94_8_1927_s_20	8873670	11  The molecule has a cell surface receptor linked by a transmembrane domain to an intracellular tyrosine kinase; it binds to heparin, basement membrane, and heparan sulfate components of the extracellular matrix, providing a tissue depot of bFGF.	bind
19936	1	6405	5	NULL	NULL	0	NULL	apo B	NULL		bind	NULL				LDL receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_963_s_128	7600129	11  The same experiment, performed without removal of free apolipoproteins, produced the same results, indicating that free apolipoproteins do not interfere with apo B binding to the LDL receptor (Fig 1  ).	bind
19937	2	6405	5	NULL	NULL	0	NULL	apolipoproteins	NULL	free	does not interfere with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_963_s_128	7600129	11  The same experiment, performed without removal of free apolipoproteins, produced the same results, indicating that free apolipoproteins do not interfere with apo B binding to the LDL receptor (Fig 1  ).	bind
23002	1	6405	7	NULL	NULL	NULL	NULL	 apo B	GP		bind					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_963_s_128	7600129	11  The same experiment, performed without removal of free apolipoproteins, produced the same results, indicating that free apolipoproteins do not interfere with apo B binding to the LDL receptor (Fig 1  ).	bind
23003	2	6405	7	NULL	NULL	NULL	NULL	apolipoproteins	GP	free	does not interfere with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_963_s_128	7600129	11  The same experiment, performed without removal of free apolipoproteins, produced the same results, indicating that free apolipoproteins do not interfere with apo B binding to the LDL receptor (Fig 1  ).	bind
19938	1	6406	5	NULL	NULL	0	NULL	SEK-1	NULL		bind	NULL				Ste5 homologues	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_78_6_947_s_46	8635244	11  Under this scenario, SEK-1, which could activate p38, never gains access to it because SEK-1 and p38 are bound to different Ste5 homologues.	bind
19939	2	6406	5	NULL	NULL	0	NULL	p38	NULL		bind	NULL				Ste5 homologues	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_78_6_947_s_46	8635244	11  Under this scenario, SEK-1, which could activate p38, never gains access to it because SEK-1 and p38 are bound to different Ste5 homologues.	bind
19940	3	6406	5	NULL	NULL	0	NULL	SEK-1	NULL		activate	NULL				p38	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_6_947_s_46	8635244	11  Under this scenario, SEK-1, which could activate p38, never gains access to it because SEK-1 and p38 are bound to different Ste5 homologues.	bind
19941	4	6406	5	NULL	NULL	0	NULL	SEK-1	NULL		does not gain access to	NULL				p38	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_6_947_s_46	8635244	11  Under this scenario, SEK-1, which could activate p38, never gains access to it because SEK-1 and p38 are bound to different Ste5 homologues.	bind
19942	5	6406	5	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_78_6_947_s_46	8635244	11  Under this scenario, SEK-1, which could activate p38, never gains access to it because SEK-1 and p38 are bound to different Ste5 homologues.	bind
19943	6	6406	5	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_78_6_947_s_46	8635244	11  Under this scenario, SEK-1, which could activate p38, never gains access to it because SEK-1 and p38 are bound to different Ste5 homologues.	bind
23004	1	6406	7	NULL	NULL	NULL	NULL	SEK-1	GP		bind					Ste5 homologue	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_6_947_s_46	8635244	11  Under this scenario, SEK-1, which could activate p38, never gains access to it because SEK-1 and p38 are bound to different Ste5 homologues.	bind
23005	2	6406	7	NULL	NULL	NULL	NULL	p38	GP		bind					Ste5 homologue	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_6_947_s_46	8635244	11  Under this scenario, SEK-1, which could activate p38, never gains access to it because SEK-1 and p38 are bound to different Ste5 homologues.	bind
23007	3	6406	7	NULL	NULL	NULL	NULL	SEK-1	GP		activate					p38	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_6_947_s_46	8635244	11  Under this scenario, SEK-1, which could activate p38, never gains access to it because SEK-1 and p38 are bound to different Ste5 homologues.	bind
30259	4	6406	7	NULL	NULL	NULL	NULL	SEK-1	GP		does not gain access to					p38	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_6_947_s_46	8635244	11  Under this scenario, SEK-1, which could activate p38, never gains access to it because SEK-1 and p38 are bound to different Ste5 homologues.	bind
30260	5	6406	7	NULL	NULL	NULL	NULL	statement 1	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_6_947_s_46	8635244	11  Under this scenario, SEK-1, which could activate p38, never gains access to it because SEK-1 and p38 are bound to different Ste5 homologues.	bind
30261	6	6406	7	NULL	NULL	NULL	NULL	statement 2	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_6_947_s_46	8635244	11  Under this scenario, SEK-1, which could activate p38, never gains access to it because SEK-1 and p38 are bound to different Ste5 homologues.	bind
19953	1	6407	5	NULL	NULL	0	NULL	Lp(a)	NULL		bind	NULL				lysine	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_5_656_s_25	8963723	11 12  Lp(a) also binds to lysine-Sepharose, 3  several cell types, including hepatocytes, 13 14  monocytes, 15  16 17  and endothelial cells, 18 19  and extracellular matrices 20  21  and matrix proteins.	bind
19954	2	6407	5	NULL	NULL	0	NULL	Lp(a)	NULL		bind	NULL				hepatocytes	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_5_656_s_25	8963723	11 12  Lp(a) also binds to lysine-Sepharose, 3  several cell types, including hepatocytes, 13 14  monocytes, 15  16 17  and endothelial cells, 18 19  and extracellular matrices 20  21  and matrix proteins.	bind
19955	3	6407	5	NULL	NULL	0	NULL	Lp(a)	NULL		bind	NULL				monocytes	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_5_656_s_25	8963723	11 12  Lp(a) also binds to lysine-Sepharose, 3  several cell types, including hepatocytes, 13 14  monocytes, 15  16 17  and endothelial cells, 18 19  and extracellular matrices 20  21  and matrix proteins.	bind
19956	4	6407	5	NULL	NULL	0	NULL	Lp(a)	NULL		bind	NULL				endothelial cells	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_5_656_s_25	8963723	11 12  Lp(a) also binds to lysine-Sepharose, 3  several cell types, including hepatocytes, 13 14  monocytes, 15  16 17  and endothelial cells, 18 19  and extracellular matrices 20  21  and matrix proteins.	bind
19957	5	6407	5	NULL	NULL	0	NULL	Lp(a)	NULL		bind	NULL				extracellular matrices	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_5_656_s_25	8963723	11 12  Lp(a) also binds to lysine-Sepharose, 3  several cell types, including hepatocytes, 13 14  monocytes, 15  16 17  and endothelial cells, 18 19  and extracellular matrices 20  21  and matrix proteins.	bind
19958	6	6407	5	NULL	NULL	0	NULL	Lp(a)	NULL		bind	NULL				matrix proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_5_656_s_25	8963723	11 12  Lp(a) also binds to lysine-Sepharose, 3  several cell types, including hepatocytes, 13 14  monocytes, 15  16 17  and endothelial cells, 18 19  and extracellular matrices 20  21  and matrix proteins.	bind
23008	1	6407	7	NULL	NULL	NULL	NULL	 Lp	GP		binds to					lysine-Sepharose	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_5_656_s_25	8963723	11 12  Lp(a) also binds to lysine-Sepharose, 3  several cell types, including hepatocytes, 13 14  monocytes, 15  16 17  and endothelial cells, 18 19  and extracellular matrices 20  21  and matrix proteins.	bind
23009	2	6407	7	NULL	NULL	NULL	NULL	Lp	GP		binds to					hepatocytes	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_5_656_s_25	8963723	11 12  Lp(a) also binds to lysine-Sepharose, 3  several cell types, including hepatocytes, 13 14  monocytes, 15  16 17  and endothelial cells, 18 19  and extracellular matrices 20  21  and matrix proteins.	bind
23010	3	6407	7	NULL	NULL	NULL	NULL	Lp	GP		binds to					monocytes	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_5_656_s_25	8963723	11 12  Lp(a) also binds to lysine-Sepharose, 3  several cell types, including hepatocytes, 13 14  monocytes, 15  16 17  and endothelial cells, 18 19  and extracellular matrices 20  21  and matrix proteins.	bind
23011	4	6407	7	NULL	NULL	NULL	NULL	Lp	GP		binds to					endothelial cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_5_656_s_25	8963723	11 12  Lp(a) also binds to lysine-Sepharose, 3  several cell types, including hepatocytes, 13 14  monocytes, 15  16 17  and endothelial cells, 18 19  and extracellular matrices 20  21  and matrix proteins.	bind
23012	5	6407	7	NULL	NULL	NULL	NULL	Lp	GP		binds to					extracellular matrices	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_5_656_s_25	8963723	11 12  Lp(a) also binds to lysine-Sepharose, 3  several cell types, including hepatocytes, 13 14  monocytes, 15  16 17  and endothelial cells, 18 19  and extracellular matrices 20  21  and matrix proteins.	bind
23013	6	6407	7	NULL	NULL	NULL	NULL	Lp	GP		binds to					matrix proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_5_656_s_25	8963723	11 12  Lp(a) also binds to lysine-Sepharose, 3  several cell types, including hepatocytes, 13 14  monocytes, 15  16 17  and endothelial cells, 18 19  and extracellular matrices 20  21  and matrix proteins.	bind
19944	1	6410	5	NULL	NULL	0	NULL	HB-EGF	NULL		bind	NULL				EGF-R	NULL				NULL	human SMCs	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1524_s_28	8977458	11 12 13  HB-EGF binds to the EGF-R of human 14  and bovine SMCs 15  and stimulates its phosphorylation.	bind
19945	2	6410	5	NULL	NULL	0	NULL	HB-EGF	NULL		bind	NULL				EGF-R	NULL				NULL	bovine SMCs	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1524_s_28	8977458	11 12 13  HB-EGF binds to the EGF-R of human 14  and bovine SMCs 15  and stimulates its phosphorylation.	bind
19946	3	6410	5	NULL	NULL	0	NULL	statement 1	NULL		stimulates	NULL				EGF-R	NULL	phosphorylation of			NULL	human SMCs	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1524_s_28	8977458	11 12 13  HB-EGF binds to the EGF-R of human 14  and bovine SMCs 15  and stimulates its phosphorylation.	bind
19947	4	6410	5	NULL	NULL	0	NULL	statement 2	NULL		stimulates	NULL				EGF-R	NULL	phosphorylation of			NULL	bovine SMCs	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1524_s_28	8977458	11 12 13  HB-EGF binds to the EGF-R of human 14  and bovine SMCs 15  and stimulates its phosphorylation.	bind
23015	1	6410	7	NULL	NULL	NULL	NULL	HB-EGF	GP		binds to					EGF-R	GP				NULL	human SMCs	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1524_s_28	8977458	11 12 13  HB-EGF binds to the EGF-R of human 14  and bovine SMCs 15  and stimulates its phosphorylation.	bind
23016	2	6410	7	NULL	NULL	NULL	NULL	HB-EGF	GP		binds to					EGF-R	GP				NULL	bovine SMCs	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1524_s_28	8977458	11 12 13  HB-EGF binds to the EGF-R of human 14  and bovine SMCs 15  and stimulates its phosphorylation.	bind
30262	3	6410	7	NULL	NULL	NULL	NULL	statement 1	Process		stimulates					EGF-R	GP	phosphorylation of			NULL	human SMCs	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1524_s_28	8977458	11 12 13  HB-EGF binds to the EGF-R of human 14  and bovine SMCs 15  and stimulates its phosphorylation.	bind
30263	4	6410	7	NULL	NULL	NULL	NULL	statement 2	Process		stimulates					EGF-R	GP	phosphorylation of			NULL	bovine SMCs	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1524_s_28	8977458	11 12 13  HB-EGF binds to the EGF-R of human 14  and bovine SMCs 15  and stimulates its phosphorylation.	bind
19948	1	6411	5	10	NULL	0	NULL	TPA			exists as					TPA		free;;active			NULL	in blood	NULL	NULL	NULL	NULL	gw60_circulation_96_3_761_s_16	9264480	11 12 13 14  TPA exists in several forms in blood, including free active TPA and TPA bound to PAI-1 and other inhibitors.	bind
19949	2	6411	5	NULL	NULL	0	NULL	TPA	NULL		bind	NULL				PAI-1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_3_761_s_16	9264480	11 12 13 14  TPA exists in several forms in blood, including free active TPA and TPA bound to PAI-1 and other inhibitors.	bind
19951	4	6411	5	NULL	NULL	0	NULL	TPA	NULL		exists as	NULL				statement 2	NULL				NULL	in blood	0	NULL	NULL	NULL	gw60_circulation_96_3_761_s_16	9264480	11 12 13 14  TPA exists in several forms in blood, including free active TPA and TPA bound to PAI-1 and other inhibitors.	bind
23017	1	6411	7	NULL	NULL	NULL	NULL	TPA 	GP		bind					PAI-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_3_761_s_16	9264480	11 12 13 14  TPA exists in several forms in blood, including free active TPA and TPA bound to PAI-1 and other inhibitors.	bind
54256	2	6411	7	NULL	NULL	NULL	NULL	TPA	GP		exists as					statement 1	Process				NULL	blood	NULL	NULL	NULL	NULL	gw60_circulation_96_3_761_s_16	9264480	11 12 13 14  TPA exists in several forms in blood, including free active TPA and TPA bound to PAI-1 and other inhibitors.	bind
54257	3	6411	7	NULL	NULL	NULL	NULL	TPA	GP		exists as					TPA	GP	free;;active			NULL	blood	NULL	NULL	NULL	NULL	gw60_circulation_96_3_761_s_16	9264480	11 12 13 14  TPA exists in several forms in blood, including free active TPA and TPA bound to PAI-1 and other inhibitors.	bind
19961	1	6412	5	NULL	NULL	0	NULL	apoB-100 	NULL		bind	NULL	strongly	LDL receptor - binding regions		GAGs	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_149_s_250	9012650	11 14  The data presented here and from other studies indicate that the LDL receptor - binding regions of apoB-100 are also the segments that bind GAGs most strongly.	bind
23018	1	6412	7	NULL	NULL	NULL	NULL	apoB-100	GP		bind		strongly	LDL receptor - binding region		GAGs	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_149_s_250	9012650	11 14  The data presented here and from other studies indicate that the LDL receptor - binding regions of apoB-100 are also the segments that bind GAGs most strongly.	bind
19962	1	6413	5	NULL	NULL	0	NULL	fibrinogen	NULL		bind	NULL				GP IIb/IIIa receptors	NULL	activated			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_954_s_202	9633937	11 22 23 24  Phillips et al 25  studied binding of PAC1, an antibody that simulates fibrinogen binding to activated GP IIb/IIIa receptors, after ADP stimulation.	bind
19963	2	6413	5	NULL	NULL	0	NULL	PAC1 antibody	NULL		stimulates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_954_s_202	9633937	11 22 23 24  Phillips et al 25  studied binding of PAC1, an antibody that simulates fibrinogen binding to activated GP IIb/IIIa receptors, after ADP stimulation.	bind
19964	3	6413	5	NULL	NULL	0	NULL	ADP	NULL	stimulation	is required for	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_954_s_202	9633937	11 22 23 24  Phillips et al 25  studied binding of PAC1, an antibody that simulates fibrinogen binding to activated GP IIb/IIIa receptors, after ADP stimulation.	bind
23019	1	6413	7	NULL	NULL	NULL	NULL	fibrinogen	GP		bind					GP IIb/IIIa receptors	GP	activated			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_954_s_202	9633937	11 22 23 24  Phillips et al 25  studied binding of PAC1, an antibody that simulates fibrinogen binding to activated GP IIb/IIIa receptors, after ADP stimulation.	bind
23020	2	6413	7	NULL	NULL	NULL	NULL	PAC1 antibody	GP		stimulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_954_s_202	9633937	11 22 23 24  Phillips et al 25  studied binding of PAC1, an antibody that simulates fibrinogen binding to activated GP IIb/IIIa receptors, after ADP stimulation.	bind
23021	3	6413	7	NULL	NULL	NULL	NULL	statement 2	Process		occurs after					ADP	Chemical	stimulation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_954_s_202	9633937	11 22 23 24  Phillips et al 25  studied binding of PAC1, an antibody that simulates fibrinogen binding to activated GP IIb/IIIa receptors, after ADP stimulation.	bind
25765	1	6414	5	NULL	NULL	0	NULL	polypeptides	NULL	protein folding of newly synthesized	is essential for	NULL				oxidative metabolism	NULL	maintaining			NULL		0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25766	2	6414	5	NULL	NULL	0	NULL	statement 1	NULL		occurs after	NULL				myocyte	NULL	damage of			NULL		0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25767	3	6414	5	NULL	NULL	0	NULL	statement 1	NULL		is a function of	NULL	potential			molecular chaperones	NULL				NULL	in ischemic heart	NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25768	4	6414	5	NULL	NULL	0	NULL	mitochondria	NULL		is protected from	NULL				ROS	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25769	5	6414	5	NULL	NULL	0	NULL	statement 4	NULL		is a function of	NULL	potential			molecular chaperones	NULL				NULL	in ischemic heart	0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25770	6	6414	5	NULL	NULL	0	NULL	TNFalpha	NULL		is a type of	NULL				cytokines	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25771	7	6414	5	NULL	NULL	0	NULL	mitochondria	NULL		is protected from	NULL				cytokines	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25772	8	6414	5	NULL	NULL	0	NULL	statement 7	NULL		is a function of	NULL	potential			molecular chaperones	NULL				NULL	in ischemic heart	0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25773	9	6414	5	NULL	NULL	0	NULL	proteins	NULL	newly synthesized	undergoes	NULL				translocation	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25774	10	6414	5	NULL	NULL	0	NULL	statement 9	NULL		occurs during	NULL				organelle repair	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25775	11	6414	5	NULL	NULL	0	NULL	statement 10	NULL		is a function of	NULL	potential			molecular chaperones	NULL				NULL	in ischemic heart	0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25776	12	6414	5	NULL	NULL	0	NULL	molecular chaperones	NULL		repairs	NULL	potential			structural proteins	NULL	critical			NULL	in ischemic heart	0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25777	13	6414	5	10	NULL	0	NULL	statement 12			occurs after					statement 37					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25778	14	6414	5	NULL	NULL	0	NULL	molecular chaperones	NULL		recycles	NULL	potential			membrane vesicles	NULL				NULL	in ischemic heart	0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25779	15	6414	5	NULL	NULL	0	NULL	molecular chaperones	NULL		transports	NULL	potential			byproducts	NULL	potential toxic			NULL	in ischemic heart	0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25780	16	6414	5	NULL	NULL	0	NULL	proteasome	NULL		degrades	NULL				byproducts	NULL	potential toxic			NULL		0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25781	17	6414	5	NULL	NULL	0	NULL	pro - interleukin-1beta	NULL		is a type of	NULL				cytokines	NULL	proinflammatory			NULL		0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25782	18	6414	5	NULL	NULL	0	NULL	molecular chaperones	NULL		suppresses	NULL	potential			cytokines	NULL	proinflammatory			NULL	in ischemic heart	0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25783	19	6414	5	NULL	NULL	0	NULL	molecular chaperones	NULL		suppresses	NULL	potential			NADPH oxidase	NULL				NULL	in ischemic heart	0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25784	20	6414	5	NULL	NULL	0	NULL	statement 19	NULL		occurs by	NULL				heat shock response	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25785	21	6414	5	NULL	NULL	0	NULL	molecular chaperones	NULL		suppresses	NULL	potential			oxidative burst	NULL				NULL	in ischemic heart	0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25786	22	6414	5	NULL	NULL	0	NULL	statement 21	NULL		occurs by	NULL				heat shock response	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25787	23	6414	5	NULL	NULL	0	NULL	molecular chaperones	NULL		prevents	NULL	potential			apoptosis	NULL				NULL	in ischemic heart	0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25788	24	6414	5	NULL	NULL	0	NULL	Hsp60	NULL		bind	NULL				cytochrome c	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25789	25	6414	5	NULL	NULL	0	NULL	Hsp70	NULL		bind	NULL				cytosolic targets	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25790	26	6414	5	NULL	NULL	0	NULL	Hsp60	NULL		is a type of	NULL				mitochondrial chaperone	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25791	27	6414	5	NULL	NULL	0	NULL	Hsp70	NULL		is a type of	NULL				mitochondrial chaperone	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25792	28	6414	5	NULL	NULL	0	NULL	statement 23	NULL		occurs through	NULL				statement 24	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25793	29	6414	5	NULL	NULL	0	NULL	statement 23	NULL		occurs through	NULL				statement 25	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25794	30	6414	5	NULL	NULL	0	NULL	statement 28	NULL		is an alternative to	NULL				statement 29	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25795	31	6414	5	NULL	NULL	0	NULL	molecular chaperones	NULL		repairs	NULL	potential			ion channel	NULL				NULL	in ischemic heart	NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25796	32	6414	5	NULL	NULL	0	NULL	Hsp47 chaperone	NULL		synthesises	NULL	potential			collagen	NULL				NULL	in ischemic heart	NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25797	33	6414	5	10	NULL	0	NULL	statement 32			occurs for					reparative fibrosis					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
25798	34	6414	5	NULL	NULL	0	NULL	molecular chaperones	NULL		modulates	NULL	potential			ischemic injury	NULL	immune-mediated			NULL	in ischemic heart	0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
29967	35	6414	5	NULL	NULL	0	NULL	NO	NULL		is produced from	NULL				HSP	NULL	inducible synthesis of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
29968	36	6414	5	NULL	NULL	0	NULL	molecular chaperones	NULL		protect	NULL				statement 35	NULL				NULL	in ischemic heart	0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
55798	37	6414	5	10	NULL	0	NULL	ischemia			induces					cytoskeleton		alterations of \t\t\t			NULL		0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
23022	1	6414	7	NULL	NULL	NULL	NULL	polypeptide	GP	protein folding of newly synthesized	maintain					oxidative metabolism 	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
23023	6	6414	7	NULL	NULL	NULL	NULL	protein	GP	newly synthesized	undergoes					translocation	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
23028	10	6414	7	NULL	NULL	NULL	NULL	heat shock response	Process		suppress					NADPH oxidase	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
23029	12	6414	7	NULL	NULL	NULL	NULL	Hsp60	GP		binds					cytochrome c	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
23030	13	6414	7	NULL	NULL	NULL	NULL	Hsp70	GP		bind					cytosolic targets	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
23031	15	6414	7	NULL	NULL	NULL	NULL	statement 14	Process		occur through					statement 12	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
23033	35	6414	7	NULL	NULL	NULL	NULL	statement 15	Process		is an alternative to					statement 16	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
23034	17	6414	7	NULL	NULL	NULL	NULL	Hsp47 chaperone	GP		synthesize					collagen	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
23035	18	6414	7	NULL	NULL	NULL	NULL	statement 17	Process		occurs for					reparative fibrosis 	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
23045	7	6414	7	NULL	NULL	NULL	NULL	ischemia	MedicalFinding		induce					cytoskeletal alterations	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
30835	3	6414	7	NULL	NULL	NULL	NULL	mitochondria 	CellComponent		is protected from					ROS	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
30836	4	6414	7	NULL	NULL	NULL	NULL	mitochondria 	CellComponent		is protected from					TNFalpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
30837	5	6414	7	NULL	NULL	NULL	NULL	TNFalpha	GP		is a type of					cytokine	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
30838	2	6414	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs after					myocyte	Cell	damage of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
30839	8	6414	7	NULL	NULL	NULL	NULL	molecular chaperones	GP		transports					potential toxic byproducts	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
30840	9	6414	7	NULL	NULL	NULL	NULL	toxic byproducts	GP		is degraded by					proteasome	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
30841	11	6414	7	NULL	NULL	NULL	NULL	heat shock response	Process		suppress					oxidative burst	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
30842	16	6414	7	NULL	NULL	NULL	NULL	statement 14	Process		occur through					statement 13	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
30843	19	6414	7	NULL	NULL	NULL	NULL	statement 1	Process		is a function of 		potentially			molecular chaperones	GP				NULL	in ischemic heart	NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
54323	20	6414	7	NULL	NULL	NULL	NULL	statement 3	Process		is a function of 		potentially			molecular chaperones	GP				NULL	in ischemic heart	NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
54324	21	6414	7	NULL	NULL	NULL	NULL	statement 4	Process		is a function of 		potentially			molecular chaperones	GP				NULL	in ischemic heart	NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
54325	22	6414	7	NULL	NULL	NULL	NULL	statement 6	Process		occur during					organelle repair	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
54326	23	6414	7	NULL	NULL	NULL	NULL	statement 6	Process		is a function of 		potentially			molecular chaperones	GP				NULL	in ischemic heart	NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
54327	24	6414	7	NULL	NULL	NULL	NULL	molecular chaperones	GP		repairs					critical structural proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
54328	25	6414	7	NULL	NULL	NULL	NULL	statement 24	Process		occurs after					statement 7	Process				NULL	in ischemic heart	NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
54329	26	6414	7	NULL	NULL	NULL	NULL	molecular chaperones	GP		recycle					membrane vesicles	CellComponent				NULL	in ischemic heart	NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
54336	27	6414	7	NULL	NULL	NULL	NULL	molecular chaperones	GP		suppress					pro - interleukin-1beta 	GP				NULL	in ischemic heart	NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
54338	28	6414	7	NULL	NULL	NULL	NULL	pro - interleukin-1beta 	GP		is a type of					proinflammatory cytokines	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
54341	29	6414	7	NULL	NULL	NULL	NULL	statement 10	Process		is a function of 		potentially			molecular chaperones	GP				NULL	in ischemic heart	NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
54344	30	6414	7	NULL	NULL	NULL	NULL	statement 11	Process		is a function of 		potentially			molecular chaperones	GP				NULL	in ischemic heart	NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
54345	31	6414	7	NULL	NULL	NULL	NULL	NO	Chemical		produced from					HSP	GP	inducible synthesis of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
54348	32	6414	7	NULL	NULL	NULL	NULL	molecular chaperones	GP		protects					statement 31	Process				NULL	in ischemic heart	NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
54349	33	6414	7	NULL	NULL	NULL	NULL	Hsp60 	GP		is a type of					mitochondrial chaperone	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
54350	34	6414	7	NULL	NULL	NULL	NULL	Hsp70	GP		is a type of					mitochondrial chaperone	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
54351	14	6414	7	NULL	NULL	NULL	NULL	molecular chaperones	GP		prevents					apoptosis	Process				NULL	in ischemic heart	NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
54353	36	6414	7	NULL	NULL	NULL	NULL	molecular chaperones	GP		repair					ion channel	CellComponent				NULL	in ischemic heart	NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
54354	37	6414	7	NULL	NULL	NULL	NULL	statement 17	Process		is a function of 		potentially			molecular chaperones	GP				NULL	in ischemic heart	NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
54363	38	6414	7	NULL	NULL	NULL	NULL	molecular chaperones	GP		modulates					 ischemic injury 	MedicalFinding	 immune-mediated			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_66	9686751	11 234 235  In physiological terms, potential functions for molecular chaperones in the ischemic heart include the following: protein folding of newly synthesized polypeptides essential for maintaining oxidative metabolism after myocyte damage (L), protection of mitochondria from ROS and cytokines such as TNFalpha 204 236  and translocation of newly synthesized proteins during organelle repair (M), repair of critical structural proteins after ischemia-induced cytoskeletal alterations (N), 237  recycling of membrane vesicles (Hsc70) (O), transport of potential toxic byproducts for degradation by the proteasome (P), 78 238 239  suppression of proinflammatory cytokines such as pro - interleukin-1beta (Q), 204 236 240  suppression of NADPH oxidase and the oxidative burst by the heat shock response (R), 241  protection by NO production from inducible synthesis of HSP expression (S), 61 242 243 244 245 246  prevention of apoptosis either through the mitochondrial chaperone Hsp60 binding of cytochrome  c and/or Hsp70 binding of cytosolic targets (T), 36 204  repair of ion channel (U), collagen synthesis by Hsp47 chaperone for reparative fibrosis (V), 180  and modulation of the immune-mediated ischemic injury (W).	bind
19959	1	6415	5	NULL	NULL	0	NULL	APLAs	NULL		bind	NULL	may			heparin-like glycosaminoglycans	NULL				NULL	on ECs	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_299	10669657	11 28  APLAs may bind to heparin-like glycosaminoglycans on ECs and thereby inhibit local antithrombin III activity.	bind
19960	2	6415	5	NULL	NULL	0	NULL	statement 1	NULL		inhibit	NULL				antithrombin III	NULL	activity of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_299	10669657	11 28  APLAs may bind to heparin-like glycosaminoglycans on ECs and thereby inhibit local antithrombin III activity.	bind
23047	1	6415	7	NULL	NULL	NULL	NULL	APLAs	GP		bind		may			heparin-like glycosaminoglycans 	Chemical				NULL	on ECs	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_299	10669657	11 28  APLAs may bind to heparin-like glycosaminoglycans on ECs and thereby inhibit local antithrombin III activity.	bind
23048	2	6415	7	NULL	NULL	NULL	NULL	statement 1	Process		inhibit					antithrombin III	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_563_s_299	10669657	11 28  APLAs may bind to heparin-like glycosaminoglycans on ECs and thereby inhibit local antithrombin III activity.	bind
29997	1	6417	5	NULL	NULL	0	NULL	T cells	NULL	activated	does not bind	NULL				CD40 construct	NULL	recombinant			NULL		0	NULL	NULL	NULL	gw60_jclininvest_97_1_196_s_6	8550833	11 different mutations were found in DNA from all 13 patients whose activated T cells failed to bind a recombinant  CD40 construct.	bind
23049	1	6417	7	NULL	NULL	NULL	NULL	T cells	Cell	activated	does not bind					CD40 construct	Cell	recombinant			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_1_196_s_6	8550833	11 different mutations were found in DNA from all 13 patients whose activated T cells failed to bind a recombinant  CD40 construct.	bind
19966	1	6418	5	NULL	NULL	0	NULL	RNA polymerase	NULL	Escherichia coli	bind	NULL				fork junction DNA	NULL			- 10 region of promoter	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2437_s_172	11410649	11 has also been used to examine the binding of  Escherichia coli RNA polymerase with the fork junction DNA containing the  - 10 region of the promoter ( 64).	bind
23050	1	6418	7	NULL	NULL	NULL	NULL	RNA polymerase	GP	Escherichia coli 	binds					fork junction DNA	NucleicAcid			 -10 region of the promoter	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2437_s_172	11410649	11 has also been used to examine the binding of  Escherichia coli RNA polymerase with the fork junction DNA containing the  - 10 region of the promoter ( 64).	bind
19967	1	6419	5	NULL	NULL	0	NULL	angiotensin II	NULL		does not bind	NULL				APJ	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_108_12_1432_s_30	12963638	11 However, angiotensin II does not bind to APJ.	bind
23051	1	6419	7	NULL	NULL	NULL	NULL	angiotensin II 	GP		does not bind					APJ	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_108_12_1432_s_30	12963638	11 However, angiotensin II does not bind to APJ.	bind
19968	1	6420	5	NULL	NULL	0	NULL	C pneumoniae	NULL	infection with	leads to	NULL				TF mRNA	NULL	increased			NULL		0	NULL	NULL	NULL	gw60_circulationres_92_4_394_s_165	12600889	11 In support, our data demonstrate that infection with  C pneumoniae leads to increased TF mRNA and protein that is associated with increased binding of Egr-1 to the SRR of the TF promoter and to the consensus Egr-1 sequence.	bind
20012	2	6420	5	NULL	NULL	0	NULL	Egr-1	NULL		bind	NULL				TF	NULL			SRR of promoter	NULL		0	NULL	NULL	NULL	gw60_circulationres_92_4_394_s_165	12600889	11 In support, our data demonstrate that infection with  C pneumoniae leads to increased TF mRNA and protein that is associated with increased binding of Egr-1 to the SRR of the TF promoter and to the consensus Egr-1 sequence.	bind
20013	3	6420	5	NULL	NULL	0	NULL	Egr-1	NULL		bind	NULL				Egr-1 sequence	NULL	consensus			NULL		0	NULL	NULL	NULL	gw60_circulationres_92_4_394_s_165	12600889	11 In support, our data demonstrate that infection with  C pneumoniae leads to increased TF mRNA and protein that is associated with increased binding of Egr-1 to the SRR of the TF promoter and to the consensus Egr-1 sequence.	bind
20014	4	6420	5	NULL	NULL	0	NULL	protein	NULL		associates with	NULL				statement 2	NULL	increased			NULL		0	NULL	NULL	NULL	gw60_circulationres_92_4_394_s_165	12600889	11 In support, our data demonstrate that infection with  C pneumoniae leads to increased TF mRNA and protein that is associated with increased binding of Egr-1 to the SRR of the TF promoter and to the consensus Egr-1 sequence.	bind
20015	5	6420	5	NULL	NULL	0	NULL	protein	NULL		associates with	NULL				statement 3	NULL	increased			NULL		0	NULL	NULL	NULL	gw60_circulationres_92_4_394_s_165	12600889	11 In support, our data demonstrate that infection with  C pneumoniae leads to increased TF mRNA and protein that is associated with increased binding of Egr-1 to the SRR of the TF promoter and to the consensus Egr-1 sequence.	bind
20016	6	6420	5	NULL	NULL	0	NULL	C pneumoniae	NULL	infection with	leads to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_92_4_394_s_165	12600889	11 In support, our data demonstrate that infection with  C pneumoniae leads to increased TF mRNA and protein that is associated with increased binding of Egr-1 to the SRR of the TF promoter and to the consensus Egr-1 sequence.	bind
20017	7	6420	5	NULL	NULL	0	NULL	C pneumoniae	NULL	infection with	leads to	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_92_4_394_s_165	12600889	11 In support, our data demonstrate that infection with  C pneumoniae leads to increased TF mRNA and protein that is associated with increased binding of Egr-1 to the SRR of the TF promoter and to the consensus Egr-1 sequence.	bind
23052	1	6420	7	NULL	NULL	NULL	NULL	C pneumoniae 	Organism		leads to					TF mRNA	NucleicAcid	increased			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_4_394_s_165	12600889	11 In support, our data demonstrate that infection with  C pneumoniae leads to increased TF mRNA and protein that is associated with increased binding of Egr-1 to the SRR of the TF promoter and to the consensus Egr-1 sequence.	bind
23053	2	6420	7	NULL	NULL	NULL	NULL	C pneumoniae 	Organism		leads to					TF protein	GP	increased			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_4_394_s_165	12600889	11 In support, our data demonstrate that infection with  C pneumoniae leads to increased TF mRNA and protein that is associated with increased binding of Egr-1 to the SRR of the TF promoter and to the consensus Egr-1 sequence.	bind
23054	3	6420	7	NULL	NULL	NULL	NULL	Egr-1	GP		bind					TF	GP			SRR in the promoter	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_4_394_s_165	12600889	11 In support, our data demonstrate that infection with  C pneumoniae leads to increased TF mRNA and protein that is associated with increased binding of Egr-1 to the SRR of the TF promoter and to the consensus Egr-1 sequence.	bind
23055	4	6420	7	NULL	NULL	NULL	NULL	Egr-1	GP		bind							consensus		Egr-1 sequence	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_4_394_s_165	12600889	11 In support, our data demonstrate that infection with  C pneumoniae leads to increased TF mRNA and protein that is associated with increased binding of Egr-1 to the SRR of the TF promoter and to the consensus Egr-1 sequence.	bind
23056	5	6420	7	NULL	NULL	NULL	NULL	statement 1	Process		increase					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_4_394_s_165	12600889	11 In support, our data demonstrate that infection with  C pneumoniae leads to increased TF mRNA and protein that is associated with increased binding of Egr-1 to the SRR of the TF promoter and to the consensus Egr-1 sequence.	bind
23057	6	6420	7	NULL	NULL	NULL	NULL	statement 1	Process		increase					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_4_394_s_165	12600889	11 In support, our data demonstrate that infection with  C pneumoniae leads to increased TF mRNA and protein that is associated with increased binding of Egr-1 to the SRR of the TF promoter and to the consensus Egr-1 sequence.	bind
23058	7	6420	7	NULL	NULL	NULL	NULL	statement 2	Process		increase					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_4_394_s_165	12600889	11 In support, our data demonstrate that infection with  C pneumoniae leads to increased TF mRNA and protein that is associated with increased binding of Egr-1 to the SRR of the TF promoter and to the consensus Egr-1 sequence.	bind
23059	8	6420	7	NULL	NULL	NULL	NULL	statement 2	Process		increase					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_4_394_s_165	12600889	11 In support, our data demonstrate that infection with  C pneumoniae leads to increased TF mRNA and protein that is associated with increased binding of Egr-1 to the SRR of the TF promoter and to the consensus Egr-1 sequence.	bind
20018	1	6421	5	NULL	NULL	0	NULL	TGF-beta1	NULL		is secreted in	NULL				inactive form	NULL	biologically			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1503_s_26	16690877	11 In vitro studies indicate that TGF-beta1 is secreted in a biologically inactive form in a complex with LAP. 11 Within the extracellular matrix, this precursor TGF-beta1 protein binds to latency TGF-binding protein (LTBP).	bind
20019	2	6421	5	NULL	NULL	0	NULL	statement 1	NULL		is in complex with	NULL				LAP	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1503_s_26	16690877	11 In vitro studies indicate that TGF-beta1 is secreted in a biologically inactive form in a complex with LAP. 11 Within the extracellular matrix, this precursor TGF-beta1 protein binds to latency TGF-binding protein (LTBP).	bind
20020	3	6421	5	NULL	NULL	0	NULL	TGF-beta1 protein	NULL	precursor	bind	NULL				LTBP	NULL				NULL	within the extracellular matrix	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1503_s_26	16690877	11 In vitro studies indicate that TGF-beta1 is secreted in a biologically inactive form in a complex with LAP. 11 Within the extracellular matrix, this precursor TGF-beta1 protein binds to latency TGF-binding protein (LTBP).	bind
20021	4	6421	5	NULL	NULL	0	NULL	LTBP	NULL		is	NULL				latency TGF-binding protein	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1503_s_26	16690877	11 In vitro studies indicate that TGF-beta1 is secreted in a biologically inactive form in a complex with LAP. 11 Within the extracellular matrix, this precursor TGF-beta1 protein binds to latency TGF-binding protein (LTBP).	bind
23087	1	6421	7	NULL	NULL	NULL	NULL	TGF-beta1	GP	inactive 	complex with					LAP	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1503_s_26	16690877	11 In vitro studies indicate that TGF-beta1 is secreted in a biologically inactive form in a complex with LAP. 11 Within the extracellular matrix, this precursor TGF-beta1 protein binds to latency TGF-binding protein (LTBP).	bind
23088	2	6421	7	NULL	NULL	NULL	NULL	TGF-beta1	GP		is secreted in					inactive form	Process	biologically			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1503_s_26	16690877	11 In vitro studies indicate that TGF-beta1 is secreted in a biologically inactive form in a complex with LAP. 11 Within the extracellular matrix, this precursor TGF-beta1 protein binds to latency TGF-binding protein (LTBP).	bind
23089	3	6421	7	NULL	NULL	NULL	NULL	TGF-beta1	GP	precursor 	binds to					LTBP	GP				NULL	extracellular matrix	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1503_s_26	16690877	11 In vitro studies indicate that TGF-beta1 is secreted in a biologically inactive form in a complex with LAP. 11 Within the extracellular matrix, this precursor TGF-beta1 protein binds to latency TGF-binding protein (LTBP).	bind
23090	4	6421	7	NULL	NULL	NULL	NULL	LTBP	GP		is					latency TGF-binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1503_s_26	16690877	11 In vitro studies indicate that TGF-beta1 is secreted in a biologically inactive form in a complex with LAP. 11 Within the extracellular matrix, this precursor TGF-beta1 protein binds to latency TGF-binding protein (LTBP).	bind
20022	1	6422	5	NULL	NULL	0	NULL	Ang II	NULL		increases	NULL				Prx1	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_28	15016729	11 Moreover, we found that Ang II also increased expression of the  paired-related homeobox gene-1, (Prx1, formerly known as MHox or Phox), and that Prx1 markedly enhanced SRF binding to CArG B in the SM alpha-actin gene in EMSA. 11 Whereas these studies significantly advanced our understanding of mechanisms whereby Ang II could increase expression of multiple CArG-dependent SMC genes, there were several unresolved questions from these studies.	bind
20023	2	6422	5	NULL	NULL	0	NULL	Prx1	NULL		is	NULL				paired-related homeobox gene-1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_28	15016729	11 Moreover, we found that Ang II also increased expression of the  paired-related homeobox gene-1, (Prx1, formerly known as MHox or Phox), and that Prx1 markedly enhanced SRF binding to CArG B in the SM alpha-actin gene in EMSA. 11 Whereas these studies significantly advanced our understanding of mechanisms whereby Ang II could increase expression of multiple CArG-dependent SMC genes, there were several unresolved questions from these studies.	bind
20024	3	6422	5	NULL	NULL	0	NULL	Prx1	NULL		is formerly known as	NULL				MHox	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_28	15016729	11 Moreover, we found that Ang II also increased expression of the  paired-related homeobox gene-1, (Prx1, formerly known as MHox or Phox), and that Prx1 markedly enhanced SRF binding to CArG B in the SM alpha-actin gene in EMSA. 11 Whereas these studies significantly advanced our understanding of mechanisms whereby Ang II could increase expression of multiple CArG-dependent SMC genes, there were several unresolved questions from these studies.	bind
20025	4	6422	5	NULL	NULL	0	NULL	Prx1	NULL		is formerly known as	NULL				Phox	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_28	15016729	11 Moreover, we found that Ang II also increased expression of the  paired-related homeobox gene-1, (Prx1, formerly known as MHox or Phox), and that Prx1 markedly enhanced SRF binding to CArG B in the SM alpha-actin gene in EMSA. 11 Whereas these studies significantly advanced our understanding of mechanisms whereby Ang II could increase expression of multiple CArG-dependent SMC genes, there were several unresolved questions from these studies.	bind
20026	5	6422	5	NULL	NULL	0	NULL	statement 3	NULL		is an alternative to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_28	15016729	11 Moreover, we found that Ang II also increased expression of the  paired-related homeobox gene-1, (Prx1, formerly known as MHox or Phox), and that Prx1 markedly enhanced SRF binding to CArG B in the SM alpha-actin gene in EMSA. 11 Whereas these studies significantly advanced our understanding of mechanisms whereby Ang II could increase expression of multiple CArG-dependent SMC genes, there were several unresolved questions from these studies.	bind
20027	6	6422	5	NULL	NULL	0	NULL	SRF	NULL		bind	NULL				SM alpha-actin gene	NULL			CArG B	NULL		0	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_28	15016729	11 Moreover, we found that Ang II also increased expression of the  paired-related homeobox gene-1, (Prx1, formerly known as MHox or Phox), and that Prx1 markedly enhanced SRF binding to CArG B in the SM alpha-actin gene in EMSA. 11 Whereas these studies significantly advanced our understanding of mechanisms whereby Ang II could increase expression of multiple CArG-dependent SMC genes, there were several unresolved questions from these studies.	bind
20028	7	6422	5	NULL	NULL	0	NULL	Prx1	NULL		enhances	NULL	markedly			statement 6	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_28	15016729	11 Moreover, we found that Ang II also increased expression of the  paired-related homeobox gene-1, (Prx1, formerly known as MHox or Phox), and that Prx1 markedly enhanced SRF binding to CArG B in the SM alpha-actin gene in EMSA. 11 Whereas these studies significantly advanced our understanding of mechanisms whereby Ang II could increase expression of multiple CArG-dependent SMC genes, there were several unresolved questions from these studies.	bind
20029	8	6422	5	10	NULL	0	NULL	Ang II	NULL		increases	NULL				SMC genes	NULL	expression of;; CArG-dependent			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_28	15016729	11 Moreover, we found that Ang II also increased expression of the  paired-related homeobox gene-1, (Prx1, formerly known as MHox or Phox), and that Prx1 markedly enhanced SRF binding to CArG B in the SM alpha-actin gene in EMSA. 11 Whereas these studies significantly advanced our understanding of mechanisms whereby Ang II could increase expression of multiple CArG-dependent SMC genes, there were several unresolved questions from these studies.	bind
23192	1	6422	7	NULL	NULL	NULL	NULL	Ang II 	GP		increase					Prx1	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_28	15016729	11 Moreover, we found that Ang II also increased expression of the  paired-related homeobox gene-1, (Prx1, formerly known as MHox or Phox), and that Prx1 markedly enhanced SRF binding to CArG B in the SM alpha-actin gene in EMSA. 11 Whereas these studies significantly advanced our understanding of mechanisms whereby Ang II could increase expression of multiple CArG-dependent SMC genes, there were several unresolved questions from these studies.	bind
23193	2	6422	7	NULL	NULL	NULL	NULL	SRF	GP		bind					SM alpha-actin gene	GP			CArG B	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_28	15016729	11 Moreover, we found that Ang II also increased expression of the  paired-related homeobox gene-1, (Prx1, formerly known as MHox or Phox), and that Prx1 markedly enhanced SRF binding to CArG B in the SM alpha-actin gene in EMSA. 11 Whereas these studies significantly advanced our understanding of mechanisms whereby Ang II could increase expression of multiple CArG-dependent SMC genes, there were several unresolved questions from these studies.	bind
23194	3	6422	7	NULL	NULL	NULL	NULL	Prx1	GP		enhance					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_28	15016729	11 Moreover, we found that Ang II also increased expression of the  paired-related homeobox gene-1, (Prx1, formerly known as MHox or Phox), and that Prx1 markedly enhanced SRF binding to CArG B in the SM alpha-actin gene in EMSA. 11 Whereas these studies significantly advanced our understanding of mechanisms whereby Ang II could increase expression of multiple CArG-dependent SMC genes, there were several unresolved questions from these studies.	bind
23195	4	6422	7	NULL	NULL	NULL	NULL	Ang II 	GP		increase					SMC genes	GP	expression of;;CArG-dependent 			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_28	15016729	11 Moreover, we found that Ang II also increased expression of the  paired-related homeobox gene-1, (Prx1, formerly known as MHox or Phox), and that Prx1 markedly enhanced SRF binding to CArG B in the SM alpha-actin gene in EMSA. 11 Whereas these studies significantly advanced our understanding of mechanisms whereby Ang II could increase expression of multiple CArG-dependent SMC genes, there were several unresolved questions from these studies.	bind
23196	5	6422	7	NULL	NULL	NULL	NULL	Prx1	GP		is					paired-related homeobox gene-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_28	15016729	11 Moreover, we found that Ang II also increased expression of the  paired-related homeobox gene-1, (Prx1, formerly known as MHox or Phox), and that Prx1 markedly enhanced SRF binding to CArG B in the SM alpha-actin gene in EMSA. 11 Whereas these studies significantly advanced our understanding of mechanisms whereby Ang II could increase expression of multiple CArG-dependent SMC genes, there were several unresolved questions from these studies.	bind
23197	6	6422	7	NULL	NULL	NULL	NULL	Prx1	GP		formerly known as					MHox	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_28	15016729	11 Moreover, we found that Ang II also increased expression of the  paired-related homeobox gene-1, (Prx1, formerly known as MHox or Phox), and that Prx1 markedly enhanced SRF binding to CArG B in the SM alpha-actin gene in EMSA. 11 Whereas these studies significantly advanced our understanding of mechanisms whereby Ang II could increase expression of multiple CArG-dependent SMC genes, there were several unresolved questions from these studies.	bind
23198	7	6422	7	NULL	NULL	NULL	NULL	Prx1	GP		formerly known as					Phox	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_28	15016729	11 Moreover, we found that Ang II also increased expression of the  paired-related homeobox gene-1, (Prx1, formerly known as MHox or Phox), and that Prx1 markedly enhanced SRF binding to CArG B in the SM alpha-actin gene in EMSA. 11 Whereas these studies significantly advanced our understanding of mechanisms whereby Ang II could increase expression of multiple CArG-dependent SMC genes, there were several unresolved questions from these studies.	bind
25972	1	6424	5	NULL	NULL	0	NULL	PGRMC1	NULL		bind	NULL				progesterone AOP2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_febslett_579_5_1089_s_193	15710396	11 Proteolysis and peptidolysis  1.37  Y12711 Rogesterone receptor membrane component 1 PGRMC1 Xq22-q24 Liver-rich protein that binds to progesterone  1.36  D14662 Anti-oxidant protein 2 AOP2 1q23.	bind
25974	2	6424	5	NULL	NULL	0	NULL	PGRMC1	NULL		is	NULL				progesterone receptor membrane component 1	NULL				NULL		0	NULL	NULL	NULL	gw70_febslett_579_5_1089_s_193	15710396	11 Proteolysis and peptidolysis  1.37  Y12711 Rogesterone receptor membrane component 1 PGRMC1 Xq22-q24 Liver-rich protein that binds to progesterone  1.36  D14662 Anti-oxidant protein 2 AOP2 1q23.	bind
25976	3	6424	5	NULL	NULL	0	NULL	AOP2	NULL		is	NULL				Anti-oxidant protein 2	NULL				NULL		0	NULL	NULL	NULL	gw70_febslett_579_5_1089_s_193	15710396	11 Proteolysis and peptidolysis  1.37  Y12711 Rogesterone receptor membrane component 1 PGRMC1 Xq22-q24 Liver-rich protein that binds to progesterone  1.36  D14662 Anti-oxidant protein 2 AOP2 1q23.	bind
23199	1	6424	7	NULL	NULL	NULL	NULL	PGRMC1	GP		binds to					progesterone AOP2	GP				NULL		NULL	NULL	NULL	NULL	gw70_febslett_579_5_1089_s_193	15710396	11 Proteolysis and peptidolysis  1.37  Y12711 Rogesterone receptor membrane component 1 PGRMC1 Xq22-q24 Liver-rich protein that binds to progesterone  1.36  D14662 Anti-oxidant protein 2 AOP2 1q23.	bind
23200	2	6424	7	NULL	NULL	NULL	NULL	PGRMC1	GP		is					Rogesterone receptor membrane component 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_febslett_579_5_1089_s_193	15710396	11 Proteolysis and peptidolysis  1.37  Y12711 Rogesterone receptor membrane component 1 PGRMC1 Xq22-q24 Liver-rich protein that binds to progesterone  1.36  D14662 Anti-oxidant protein 2 AOP2 1q23.	bind
23201	3	6424	7	NULL	NULL	NULL	NULL	AOP2	GP		is					Anti-oxidant protein 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_febslett_579_5_1089_s_193	15710396	11 Proteolysis and peptidolysis  1.37  Y12711 Rogesterone receptor membrane component 1 PGRMC1 Xq22-q24 Liver-rich protein that binds to progesterone  1.36  D14662 Anti-oxidant protein 2 AOP2 1q23.	bind
20070	1	6425	5	NULL	NULL	0	NULL	Ang II	NULL	induced	increases	NULL				SM alpha-actin	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_185	15016729	11 Results thus support a model wherein Ang II-induced increases SM alpha-actin expression are mediated through Prx1-mediated increases in SRF binding to degenerate CArG elements and subsequent recruitment of myocardin and/or other SRF coactivators.	bind
20071	2	6425	5	NULL	NULL	0	NULL	SRF	NULL		bind	NULL					NULL	degenerate		CArG elements	NULL		0	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_185	15016729	11 Results thus support a model wherein Ang II-induced increases SM alpha-actin expression are mediated through Prx1-mediated increases in SRF binding to degenerate CArG elements and subsequent recruitment of myocardin and/or other SRF coactivators.	bind
20072	3	6425	5	NULL	NULL	0	NULL	statement 2	NULL		recruits	NULL	subsequently			myocardin	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_185	15016729	11 Results thus support a model wherein Ang II-induced increases SM alpha-actin expression are mediated through Prx1-mediated increases in SRF binding to degenerate CArG elements and subsequent recruitment of myocardin and/or other SRF coactivators.	bind
20073	4	6425	5	NULL	NULL	0	NULL	statement 2	NULL		recruits	NULL	subsequently			SRF coactivators	NULL	other			NULL		0	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_185	15016729	11 Results thus support a model wherein Ang II-induced increases SM alpha-actin expression are mediated through Prx1-mediated increases in SRF binding to degenerate CArG elements and subsequent recruitment of myocardin and/or other SRF coactivators.	bind
20074	5	6425	5	NULL	NULL	0	NULL	Prx1	NULL		mediate	NULL				statement 2	NULL	increase in			NULL		0	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_185	15016729	11 Results thus support a model wherein Ang II-induced increases SM alpha-actin expression are mediated through Prx1-mediated increases in SRF binding to degenerate CArG elements and subsequent recruitment of myocardin and/or other SRF coactivators.	bind
20075	6	6425	5	NULL	NULL	0	NULL	Prx1	NULL		mediate	NULL				statement 3	NULL	increase in			NULL		0	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_185	15016729	11 Results thus support a model wherein Ang II-induced increases SM alpha-actin expression are mediated through Prx1-mediated increases in SRF binding to degenerate CArG elements and subsequent recruitment of myocardin and/or other SRF coactivators.	bind
20076	7	6425	5	NULL	NULL	0	NULL	Prx1	NULL		mediate	NULL				statement 4	NULL	increase in			NULL		0	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_185	15016729	11 Results thus support a model wherein Ang II-induced increases SM alpha-actin expression are mediated through Prx1-mediated increases in SRF binding to degenerate CArG elements and subsequent recruitment of myocardin and/or other SRF coactivators.	bind
20077	8	6425	5	NULL	NULL	0	NULL	statement 1	NULL		is mediated through	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_185	15016729	11 Results thus support a model wherein Ang II-induced increases SM alpha-actin expression are mediated through Prx1-mediated increases in SRF binding to degenerate CArG elements and subsequent recruitment of myocardin and/or other SRF coactivators.	bind
20078	9	6425	5	NULL	NULL	0	NULL	statement 1	NULL		is mediated through	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_185	15016729	11 Results thus support a model wherein Ang II-induced increases SM alpha-actin expression are mediated through Prx1-mediated increases in SRF binding to degenerate CArG elements and subsequent recruitment of myocardin and/or other SRF coactivators.	bind
20079	10	6425	5	NULL	NULL	0	NULL	statement 1	NULL		is mediated through	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_185	15016729	11 Results thus support a model wherein Ang II-induced increases SM alpha-actin expression are mediated through Prx1-mediated increases in SRF binding to degenerate CArG elements and subsequent recruitment of myocardin and/or other SRF coactivators.	bind
23202	1	6425	7	NULL	NULL	NULL	NULL	Ang II	GP	induced	increase					SM alpha-actin	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_185	15016729	11 Results thus support a model wherein Ang II-induced increases SM alpha-actin expression are mediated through Prx1-mediated increases in SRF binding to degenerate CArG elements and subsequent recruitment of myocardin and/or other SRF coactivators.	bind
23203	2	6425	7	NULL	NULL	NULL	NULL	 SRF	GP		bind									CArG elements 	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_185	15016729	11 Results thus support a model wherein Ang II-induced increases SM alpha-actin expression are mediated through Prx1-mediated increases in SRF binding to degenerate CArG elements and subsequent recruitment of myocardin and/or other SRF coactivators.	bind
23204	3	6425	7	NULL	NULL	NULL	NULL	statement 2	Process		degenerate									CArG elements 	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_185	15016729	11 Results thus support a model wherein Ang II-induced increases SM alpha-actin expression are mediated through Prx1-mediated increases in SRF binding to degenerate CArG elements and subsequent recruitment of myocardin and/or other SRF coactivators.	bind
23205	4	6425	7	NULL	NULL	NULL	NULL	Prx-1	GP		mediates					statement 2	Process	increase in			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_185	15016729	11 Results thus support a model wherein Ang II-induced increases SM alpha-actin expression are mediated through Prx1-mediated increases in SRF binding to degenerate CArG elements and subsequent recruitment of myocardin and/or other SRF coactivators.	bind
23206	5	6425	7	NULL	NULL	NULL	NULL	statement 2	Process		recruits					myocardin	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_185	15016729	11 Results thus support a model wherein Ang II-induced increases SM alpha-actin expression are mediated through Prx1-mediated increases in SRF binding to degenerate CArG elements and subsequent recruitment of myocardin and/or other SRF coactivators.	bind
23207	6	6425	7	NULL	NULL	NULL	NULL	statement 2	GP		recruits					SRF coactivators	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_185	15016729	11 Results thus support a model wherein Ang II-induced increases SM alpha-actin expression are mediated through Prx1-mediated increases in SRF binding to degenerate CArG elements and subsequent recruitment of myocardin and/or other SRF coactivators.	bind
23208	7	6425	7	NULL	NULL	NULL	NULL	statement 4	Process		mediates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_185	15016729	11 Results thus support a model wherein Ang II-induced increases SM alpha-actin expression are mediated through Prx1-mediated increases in SRF binding to degenerate CArG elements and subsequent recruitment of myocardin and/or other SRF coactivators.	bind
23209	8	6425	7	NULL	NULL	NULL	NULL	statement 5	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1075_s_185	15016729	11 Results thus support a model wherein Ang II-induced increases SM alpha-actin expression are mediated through Prx1-mediated increases in SRF binding to degenerate CArG elements and subsequent recruitment of myocardin and/or other SRF coactivators.	bind
20032	1	6426	5	NULL	NULL	0	NULL	R-L3	NULL		bind	NULL				KCNQ1 channels	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_93_10_941_s_41	14576198	11 The mechanisms of R-L3 binding and modulation of KCNQ1 channels are not understood.	bind
20033	2	6426	5	NULL	NULL	0	NULL	R-L3	NULL		modulate	NULL				KCNQ1 channels	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_93_10_941_s_41	14576198	11 The mechanisms of R-L3 binding and modulation of KCNQ1 channels are not understood.	bind
23837	1	6426	7	NULL	NULL	NULL	NULL	R-L3	Chemical		bind					KCNQ1 channels	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_10_941_s_41	14576198	11 The mechanisms of R-L3 binding and modulation of KCNQ1 channels are not understood.	bind
23838	2	6426	7	NULL	NULL	NULL	NULL	R-L3	Chemical		modulates					KCNQ1 channels	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_10_941_s_41	14576198	11 The mechanisms of R-L3 binding and modulation of KCNQ1 channels are not understood.	bind
20080	1	6427	5	NULL	NULL	0	NULL	NFATc1	NULL		bind	NULL	sequence specific			bcl-2	NULL			NFAT site within promoter	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1492_s_186	15117818	11 The present study demonstrated that NFATc1 binds to the NFAT site within the bcl-2 promoter in a sequence-specific manner.	bind
23210	1	6427	7	NULL	NULL	NULL	NULL	NFATc1	GP		binds		sequence specific			bcl-2	GP			NFAT site within the promoter	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1492_s_186	15117818	11 The present study demonstrated that NFATc1 binds to the NFAT site within the bcl-2 promoter in a sequence-specific manner.	bind
20081	1	6428	5	NULL	NULL	0	NULL	ECSOD	NULL		bind	NULL		R213G		aortic endothelial cells	NULL	bovine			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_circulation_112_7_1047_s_161	16087794	11 Third, ECSODR213G binds to bovine aortic endothelial cells 50-fold less than ECSOD in vitro, as quantified by ELISA.	bind
20082	2	6428	5	NULL	NULL	0	NULL	ECSOD	NULL		bind	NULL				aortic endothelial cells	NULL	bovine			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_circulation_112_7_1047_s_161	16087794	11 Third, ECSODR213G binds to bovine aortic endothelial cells 50-fold less than ECSOD in vitro, as quantified by ELISA.	bind
20083	3	6428	5	NULL	NULL	0	NULL	statement 1	NULL		is lesser than	NULL				statement 2	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_circulation_112_7_1047_s_161	16087794	11 Third, ECSODR213G binds to bovine aortic endothelial cells 50-fold less than ECSOD in vitro, as quantified by ELISA.	bind
23212	1	6428	7	NULL	NULL	NULL	NULL	ECSOD	GP		binds to			R213G		aortic endothelial cells	Cell	bovine			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_circulation_112_7_1047_s_161	16087794	11 Third, ECSODR213G binds to bovine aortic endothelial cells 50-fold less than ECSOD in vitro, as quantified by ELISA.	bind
23213	2	6428	7	NULL	NULL	NULL	NULL	ECSOD	GP		binds					aortic endothelial cells	Cell	bovine			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_circulation_112_7_1047_s_161	16087794	11 Third, ECSODR213G binds to bovine aortic endothelial cells 50-fold less than ECSOD in vitro, as quantified by ELISA.	bind
23214	3	6428	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs less than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_7_1047_s_161	16087794	11 Third, ECSODR213G binds to bovine aortic endothelial cells 50-fold less than ECSOD in vitro, as quantified by ELISA.	bind
20084	1	6429	5	NULL	NULL	0	NULL	AT III	NULL		is	NULL				antithrombin III	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_4_1383_s_19	11583966	11, 12  In terms of anticoagulant factors, serum levels of antithrombin III (AT III), which binds and irreversibly inactivates a number of activated serine proteases, including thrombin, are reduced in patients with acute respiratory distress syndrome.	bind
20085	2	6429	5	NULL	NULL	0	NULL	AT III	NULL		bind	NULL				serine proteases	NULL	activated			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_4_1383_s_19	11583966	11, 12  In terms of anticoagulant factors, serum levels of antithrombin III (AT III), which binds and irreversibly inactivates a number of activated serine proteases, including thrombin, are reduced in patients with acute respiratory distress syndrome.	bind
20086	3	6429	5	NULL	NULL	0	NULL	AT III	NULL		bind	NULL				thrombin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_4_1383_s_19	11583966	11, 12  In terms of anticoagulant factors, serum levels of antithrombin III (AT III), which binds and irreversibly inactivates a number of activated serine proteases, including thrombin, are reduced in patients with acute respiratory distress syndrome.	bind
20087	4	6429	5	NULL	NULL	0	NULL	statement 2	NULL		inactivates	NULL	irreversibly			serine proteases	NULL	activated			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_4_1383_s_19	11583966	11, 12  In terms of anticoagulant factors, serum levels of antithrombin III (AT III), which binds and irreversibly inactivates a number of activated serine proteases, including thrombin, are reduced in patients with acute respiratory distress syndrome.	bind
20089	6	6429	5	NULL	NULL	0	NULL	AT III	NULL	serum levels of	is reduced in	NULL				acute respiratory distress syndrome	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_4_1383_s_19	11583966	11, 12  In terms of anticoagulant factors, serum levels of antithrombin III (AT III), which binds and irreversibly inactivates a number of activated serine proteases, including thrombin, are reduced in patients with acute respiratory distress syndrome.	bind
29999	5	6429	5	NULL	NULL	0	NULL	statement 3	NULL		inactivates	NULL	irreversibly			thrombin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_4_1383_s_19	11583966	11, 12  In terms of anticoagulant factors, serum levels of antithrombin III (AT III), which binds and irreversibly inactivates a number of activated serine proteases, including thrombin, are reduced in patients with acute respiratory distress syndrome.	bind
23215	1	6429	7	NULL	NULL	NULL	NULL	AT III	GP		binds					serine proteases	GP	activated			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_4_1383_s_19	11583966	11, 12  In terms of anticoagulant factors, serum levels of antithrombin III (AT III), which binds and irreversibly inactivates a number of activated serine proteases, including thrombin, are reduced in patients with acute respiratory distress syndrome.	bind
23216	2	6429	7	NULL	NULL	NULL	NULL	AT III	GP		binds					thrombin	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_4_1383_s_19	11583966	11, 12  In terms of anticoagulant factors, serum levels of antithrombin III (AT III), which binds and irreversibly inactivates a number of activated serine proteases, including thrombin, are reduced in patients with acute respiratory distress syndrome.	bind
23217	3	6429	7	NULL	NULL	NULL	NULL	statement 1	Process		inactivates		irreversibly			serine proteases	GP	activated			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_4_1383_s_19	11583966	11, 12  In terms of anticoagulant factors, serum levels of antithrombin III (AT III), which binds and irreversibly inactivates a number of activated serine proteases, including thrombin, are reduced in patients with acute respiratory distress syndrome.	bind
23218	4	6429	7	NULL	NULL	NULL	NULL	statement 2	Process		inactivates					thrombin	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_4_1383_s_19	11583966	11, 12  In terms of anticoagulant factors, serum levels of antithrombin III (AT III), which binds and irreversibly inactivates a number of activated serine proteases, including thrombin, are reduced in patients with acute respiratory distress syndrome.	bind
23219	5	6429	7	NULL	NULL	NULL	NULL	AT III	GP		is					antithrombin III	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_4_1383_s_19	11583966	11, 12  In terms of anticoagulant factors, serum levels of antithrombin III (AT III), which binds and irreversibly inactivates a number of activated serine proteases, including thrombin, are reduced in patients with acute respiratory distress syndrome.	bind
30689	6	6429	7	NULL	NULL	NULL	NULL	ATIII	GP	serum levels of 	is reduced in					acute respiratory distress syndrome	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_4_1383_s_19	11583966	11, 12  In terms of anticoagulant factors, serum levels of antithrombin III (AT III), which binds and irreversibly inactivates a number of activated serine proteases, including thrombin, are reduced in patients with acute respiratory distress syndrome.	bind
20136	1	6431	5	NULL	NULL	0	NULL	LPS	NULL		induces	NULL				cellular responses	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_20_2608_s_179	12427659	11, 15, 27 It has been proposed that the cellular responses induced by LPS occur through the binding of LPS to CD14, with subsequent signal transduction via TLR4.	bind
20137	2	6431	5	NULL	NULL	0	NULL	LPS	NULL		bind	NULL				CD14	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_20_2608_s_179	12427659	11, 15, 27 It has been proposed that the cellular responses induced by LPS occur through the binding of LPS to CD14, with subsequent signal transduction via TLR4.	bind
20138	3	6431	5	NULL	NULL	0	NULL	statement 1	NULL		occurs through	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_20_2608_s_179	12427659	11, 15, 27 It has been proposed that the cellular responses induced by LPS occur through the binding of LPS to CD14, with subsequent signal transduction via TLR4.	bind
20139	4	6431	5	NULL	NULL	0	NULL	statement 3	NULL		occurs with	NULL	subsequently			signal transduction	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_20_2608_s_179	12427659	11, 15, 27 It has been proposed that the cellular responses induced by LPS occur through the binding of LPS to CD14, with subsequent signal transduction via TLR4.	bind
20140	5	6431	5	NULL	NULL	0	NULL	statement 4	NULL		via	NULL				TLR4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_20_2608_s_179	12427659	11, 15, 27 It has been proposed that the cellular responses induced by LPS occur through the binding of LPS to CD14, with subsequent signal transduction via TLR4.	bind
23220	1	6431	7	NULL	NULL	NULL	NULL	LPS	Chemical		bind					CD14	Cell				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_20_2608_s_179	12427659	11, 15, 27 It has been proposed that the cellular responses induced by LPS occur through the binding of LPS to CD14, with subsequent signal transduction via TLR4.	bind
23221	2	6431	7	NULL	NULL	NULL	NULL	LPS	Chemical		induce					cellular response	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_20_2608_s_179	12427659	11, 15, 27 It has been proposed that the cellular responses induced by LPS occur through the binding of LPS to CD14, with subsequent signal transduction via TLR4.	bind
23222	3	6431	7	NULL	NULL	NULL	NULL	statement 3	Process		occurs with					signal transduction	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_20_2608_s_179	12427659	11, 15, 27 It has been proposed that the cellular responses induced by LPS occur through the binding of LPS to CD14, with subsequent signal transduction via TLR4.	bind
23223	4	6431	7	NULL	NULL	NULL	NULL	statement 3	Process		occurs via					TLR4	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_20_2608_s_179	12427659	11, 15, 27 It has been proposed that the cellular responses induced by LPS occur through the binding of LPS to CD14, with subsequent signal transduction via TLR4.	bind
20141	1	6432	5	10	NULL	0	NULL				plays a role in		major		CRE	statement 8					NULL	osteoblasts	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1415_s_161	12231559	11, 16 Previous reports have indicated that CRE, CCAAT/enhancer binding protein-beta (same as NF-IL6), and activator protein-1 motifs play major roles in the shear stress induction of the COX-2 gene in osteoblasts, which is consistent with our results because of multiple binding activity of the CRE for CRE binding protein, CCAAT/enhancer binding proteins, and activator protein-1.	bind
20142	2	6432	5	10	NULL	0	NULL	CCAAT/enhancer binding protein-beta			is a synonym of					NF-IL6					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1415_s_161	12231559	11, 16 Previous reports have indicated that CRE, CCAAT/enhancer binding protein-beta (same as NF-IL6), and activator protein-1 motifs play major roles in the shear stress induction of the COX-2 gene in osteoblasts, which is consistent with our results because of multiple binding activity of the CRE for CRE binding protein, CCAAT/enhancer binding proteins, and activator protein-1.	bind
20143	3	6432	5	10	NULL	0	NULL	CCAAT/enhancer binding protein-beta			plays a role in		major			statement 8					NULL	osteoblasts	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1415_s_161	12231559	11, 16 Previous reports have indicated that CRE, CCAAT/enhancer binding protein-beta (same as NF-IL6), and activator protein-1 motifs play major roles in the shear stress induction of the COX-2 gene in osteoblasts, which is consistent with our results because of multiple binding activity of the CRE for CRE binding protein, CCAAT/enhancer binding proteins, and activator protein-1.	bind
20144	4	6432	5	10	NULL	0	NULL	activator protein-1			plays a role in		major			statement 8					NULL	osteoblasts	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1415_s_161	12231559	11, 16 Previous reports have indicated that CRE, CCAAT/enhancer binding protein-beta (same as NF-IL6), and activator protein-1 motifs play major roles in the shear stress induction of the COX-2 gene in osteoblasts, which is consistent with our results because of multiple binding activity of the CRE for CRE binding protein, CCAAT/enhancer binding proteins, and activator protein-1.	bind
20145	5	6432	5	NULL	NULL	0	NULL		NULL		bind	NULL			CRE	CRE binding protein	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1415_s_161	12231559	11, 16 Previous reports have indicated that CRE, CCAAT/enhancer binding protein-beta (same as NF-IL6), and activator protein-1 motifs play major roles in the shear stress induction of the COX-2 gene in osteoblasts, which is consistent with our results because of multiple binding activity of the CRE for CRE binding protein, CCAAT/enhancer binding proteins, and activator protein-1.	bind
20146	6	6432	5	NULL	NULL	0	NULL		NULL		bind	NULL			CRE	CCAAT/enhancer binding proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1415_s_161	12231559	11, 16 Previous reports have indicated that CRE, CCAAT/enhancer binding protein-beta (same as NF-IL6), and activator protein-1 motifs play major roles in the shear stress induction of the COX-2 gene in osteoblasts, which is consistent with our results because of multiple binding activity of the CRE for CRE binding protein, CCAAT/enhancer binding proteins, and activator protein-1.	bind
20147	7	6432	5	NULL	NULL	0	NULL		NULL		bind	NULL			CRE	activator protein-1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1415_s_161	12231559	11, 16 Previous reports have indicated that CRE, CCAAT/enhancer binding protein-beta (same as NF-IL6), and activator protein-1 motifs play major roles in the shear stress induction of the COX-2 gene in osteoblasts, which is consistent with our results because of multiple binding activity of the CRE for CRE binding protein, CCAAT/enhancer binding proteins, and activator protein-1.	bind
54258	8	6432	5	10	NULL	0	NULL	shear stress			induces					COX-2 gene					NULL	osteoblasts	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1415_s_161	12231559	11, 16 Previous reports have indicated that CRE, CCAAT/enhancer binding protein-beta (same as NF-IL6), and activator protein-1 motifs play major roles in the shear stress induction of the COX-2 gene in osteoblasts, which is consistent with our results because of multiple binding activity of the CRE for CRE binding protein, CCAAT/enhancer binding proteins, and activator protein-1.	bind
23340	1	6432	7	NULL	NULL	NULL	NULL	shear stress 	Process		induce					COX-2 gene	GP				NULL	in osteoblasts	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1415_s_161	12231559	11, 16 Previous reports have indicated that CRE, CCAAT/enhancer binding protein-beta (same as NF-IL6), and activator protein-1 motifs play major roles in the shear stress induction of the COX-2 gene in osteoblasts, which is consistent with our results because of multiple binding activity of the CRE for CRE binding protein, CCAAT/enhancer binding proteins, and activator protein-1.	bind
23342	2	6432	7	NULL	NULL	NULL	NULL				plays a role in		major		 CRE	statement 1	Process				NULL	osteoblasts	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1415_s_161	12231559	11, 16 Previous reports have indicated that CRE, CCAAT/enhancer binding protein-beta (same as NF-IL6), and activator protein-1 motifs play major roles in the shear stress induction of the COX-2 gene in osteoblasts, which is consistent with our results because of multiple binding activity of the CRE for CRE binding protein, CCAAT/enhancer binding proteins, and activator protein-1.	bind
23344	3	6432	7	NULL	NULL	NULL	NULL	CCAAT/enhancer binding protein-beta	GP		plays a role in		major			statement 1	Process				NULL	osteoblasts	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1415_s_161	12231559	11, 16 Previous reports have indicated that CRE, CCAAT/enhancer binding protein-beta (same as NF-IL6), and activator protein-1 motifs play major roles in the shear stress induction of the COX-2 gene in osteoblasts, which is consistent with our results because of multiple binding activity of the CRE for CRE binding protein, CCAAT/enhancer binding proteins, and activator protein-1.	bind
23348	4	6432	7	NULL	NULL	NULL	NULL	activator protein-1 motif	GP		plays a role in		major			statement 1	Process				NULL	osteoblasts	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1415_s_161	12231559	11, 16 Previous reports have indicated that CRE, CCAAT/enhancer binding protein-beta (same as NF-IL6), and activator protein-1 motifs play major roles in the shear stress induction of the COX-2 gene in osteoblasts, which is consistent with our results because of multiple binding activity of the CRE for CRE binding protein, CCAAT/enhancer binding proteins, and activator protein-1.	bind
23352	5	6432	7	NULL	NULL	NULL	NULL	CRE binding protein	GP		bind									CRE	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1415_s_161	12231559	11, 16 Previous reports have indicated that CRE, CCAAT/enhancer binding protein-beta (same as NF-IL6), and activator protein-1 motifs play major roles in the shear stress induction of the COX-2 gene in osteoblasts, which is consistent with our results because of multiple binding activity of the CRE for CRE binding protein, CCAAT/enhancer binding proteins, and activator protein-1.	bind
23355	6	6432	7	NULL	NULL	NULL	NULL	CCAAT/enhancer binding protein	GP		bind									CRE	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1415_s_161	12231559	11, 16 Previous reports have indicated that CRE, CCAAT/enhancer binding protein-beta (same as NF-IL6), and activator protein-1 motifs play major roles in the shear stress induction of the COX-2 gene in osteoblasts, which is consistent with our results because of multiple binding activity of the CRE for CRE binding protein, CCAAT/enhancer binding proteins, and activator protein-1.	bind
23357	7	6432	7	NULL	NULL	NULL	NULL	 activator protein-1	GP		bind									CRE	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1415_s_161	12231559	11, 16 Previous reports have indicated that CRE, CCAAT/enhancer binding protein-beta (same as NF-IL6), and activator protein-1 motifs play major roles in the shear stress induction of the COX-2 gene in osteoblasts, which is consistent with our results because of multiple binding activity of the CRE for CRE binding protein, CCAAT/enhancer binding proteins, and activator protein-1.	bind
23358	8	6432	7	NULL	NULL	NULL	NULL	CCAAT/enhancer binding protein-beta	GP		is a synonym of					NF-IL6	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1415_s_161	12231559	11, 16 Previous reports have indicated that CRE, CCAAT/enhancer binding protein-beta (same as NF-IL6), and activator protein-1 motifs play major roles in the shear stress induction of the COX-2 gene in osteoblasts, which is consistent with our results because of multiple binding activity of the CRE for CRE binding protein, CCAAT/enhancer binding proteins, and activator protein-1.	bind
20148	1	6433	5	NULL	NULL	0	NULL	Grb2	NULL		bind	NULL				Shc	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_5_1759_s_228	10550332	11, 28, 29 Our data demonstrating increased binding of adapter protein Grb2 to Shc and to Sos indicate their involvement as mediators of receptor tyrosine kinase signaling via Ras during ulcer healing.	bind
20149	2	6433	5	NULL	NULL	0	NULL	Grb2	NULL		bind	NULL				Sos	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_5_1759_s_228	10550332	11, 28, 29 Our data demonstrating increased binding of adapter protein Grb2 to Shc and to Sos indicate their involvement as mediators of receptor tyrosine kinase signaling via Ras during ulcer healing.	bind
20150	3	6433	5	NULL	NULL	0	NULL	Grb2	NULL		mediates	NULL				receptor tyrosine kinase signaling	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_5_1759_s_228	10550332	11, 28, 29 Our data demonstrating increased binding of adapter protein Grb2 to Shc and to Sos indicate their involvement as mediators of receptor tyrosine kinase signaling via Ras during ulcer healing.	bind
20151	4	6433	5	NULL	NULL	0	NULL	statement 3	NULL		via	NULL				Ras	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_5_1759_s_228	10550332	11, 28, 29 Our data demonstrating increased binding of adapter protein Grb2 to Shc and to Sos indicate their involvement as mediators of receptor tyrosine kinase signaling via Ras during ulcer healing.	bind
20152	5	6433	5	NULL	NULL	0	NULL	statement 1	NULL	increased	indicates	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_5_1759_s_228	10550332	11, 28, 29 Our data demonstrating increased binding of adapter protein Grb2 to Shc and to Sos indicate their involvement as mediators of receptor tyrosine kinase signaling via Ras during ulcer healing.	bind
20153	6	6433	5	NULL	NULL	0	NULL	statement 2	NULL	increased	indicates	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_5_1759_s_228	10550332	11, 28, 29 Our data demonstrating increased binding of adapter protein Grb2 to Shc and to Sos indicate their involvement as mediators of receptor tyrosine kinase signaling via Ras during ulcer healing.	bind
30019	7	6433	5	NULL	NULL	0	NULL	statement 3	NULL		occurs during	NULL				ulcer	NULL	healing of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_5_1759_s_228	10550332	11, 28, 29 Our data demonstrating increased binding of adapter protein Grb2 to Shc and to Sos indicate their involvement as mediators of receptor tyrosine kinase signaling via Ras during ulcer healing.	bind
30021	8	6433	5	NULL	NULL	0	NULL	Grb2	NULL		is a type of	NULL				adapter protein	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_5_1759_s_228	10550332	11, 28, 29 Our data demonstrating increased binding of adapter protein Grb2 to Shc and to Sos indicate their involvement as mediators of receptor tyrosine kinase signaling via Ras during ulcer healing.	bind
23361	1	6433	7	NULL	NULL	NULL	NULL	Grb2 	GP		bind					Shc	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_5_1759_s_228	10550332	11, 28, 29 Our data demonstrating increased binding of adapter protein Grb2 to Shc and to Sos indicate their involvement as mediators of receptor tyrosine kinase signaling via Ras during ulcer healing.	bind
23362	2	6433	7	NULL	NULL	NULL	NULL	Grb2 	GP		bind					Sos	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_5_1759_s_228	10550332	11, 28, 29 Our data demonstrating increased binding of adapter protein Grb2 to Shc and to Sos indicate their involvement as mediators of receptor tyrosine kinase signaling via Ras during ulcer healing.	bind
23363	3	6433	7	NULL	NULL	NULL	NULL	Grb2 	GP		mediates					tyrosine kinase signaling	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_5_1759_s_228	10550332	11, 28, 29 Our data demonstrating increased binding of adapter protein Grb2 to Shc and to Sos indicate their involvement as mediators of receptor tyrosine kinase signaling via Ras during ulcer healing.	bind
23364	4	6433	7	NULL	NULL	NULL	NULL	statement 3	Process		occurs via					Ras	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_5_1759_s_228	10550332	11, 28, 29 Our data demonstrating increased binding of adapter protein Grb2 to Shc and to Sos indicate their involvement as mediators of receptor tyrosine kinase signaling via Ras during ulcer healing.	bind
23365	5	6433	7	NULL	NULL	NULL	NULL	statement 3	Process		occur during					Ulcer 	MedicalFinding	healing of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_5_1759_s_228	10550332	11, 28, 29 Our data demonstrating increased binding of adapter protein Grb2 to Shc and to Sos indicate their involvement as mediators of receptor tyrosine kinase signaling via Ras during ulcer healing.	bind
54259	6	6433	7	NULL	NULL	NULL	NULL	Grb2	GP		is a type of					adapter protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_5_1759_s_228	10550332	11, 28, 29 Our data demonstrating increased binding of adapter protein Grb2 to Shc and to Sos indicate their involvement as mediators of receptor tyrosine kinase signaling via Ras during ulcer healing.	bind
20154	1	6434	5	NULL	NULL	0	NULL	FoxA1	NULL		bind	NULL					NULL			MMTV LTR	NULL		NULL	NULL	NULL	NULL	gw70_nature_435_7044_944_s_142	15959514	11, 281 285 (2000) |  PubMed |  ChemPort |            Holmqvist, P. H., Belikov, S., Zaret, K. S. & Wrange, O. FoxA1 binding to the  MMTV LTR modulates chromatin structure and transcription.	bind
20155	2	6434	5	NULL	NULL	0	NULL	statement 1	NULL		modulates	NULL				chromatin	NULL	structure of			NULL		0	NULL	NULL	NULL	gw70_nature_435_7044_944_s_142	15959514	11, 281 285 (2000) |  PubMed |  ChemPort |            Holmqvist, P. H., Belikov, S., Zaret, K. S. & Wrange, O. FoxA1 binding to the  MMTV LTR modulates chromatin structure and transcription.	bind
20156	3	6434	5	NULL	NULL	0	NULL	statement 1	NULL		modulates	NULL				transcription	NULL				NULL		0	NULL	NULL	NULL	gw70_nature_435_7044_944_s_142	15959514	11, 281 285 (2000) |  PubMed |  ChemPort |            Holmqvist, P. H., Belikov, S., Zaret, K. S. & Wrange, O. FoxA1 binding to the  MMTV LTR modulates chromatin structure and transcription.	bind
23366	1	6434	7	NULL	NULL	NULL	NULL	FoxA1	GP		binds to									MMTV LTR	NULL		NULL	NULL	NULL	NULL	gw70_nature_435_7044_944_s_142	15959514	11, 281 285 (2000) |  PubMed |  ChemPort |            Holmqvist, P. H., Belikov, S., Zaret, K. S. & Wrange, O. FoxA1 binding to the  MMTV LTR modulates chromatin structure and transcription.	bind
23367	2	6434	7	NULL	NULL	NULL	NULL	statement 1	Process		modulate					chromatin	Chromosome	structure of			NULL		NULL	NULL	NULL	NULL	gw70_nature_435_7044_944_s_142	15959514	11, 281 285 (2000) |  PubMed |  ChemPort |            Holmqvist, P. H., Belikov, S., Zaret, K. S. & Wrange, O. FoxA1 binding to the  MMTV LTR modulates chromatin structure and transcription.	bind
23368	3	6434	7	NULL	NULL	NULL	NULL	statement 1	Process		modulate					transcription	Process				NULL		NULL	NULL	NULL	NULL	gw70_nature_435_7044_944_s_142	15959514	11, 281 285 (2000) |  PubMed |  ChemPort |            Holmqvist, P. H., Belikov, S., Zaret, K. S. & Wrange, O. FoxA1 binding to the  MMTV LTR modulates chromatin structure and transcription.	bind
20157	1	6435	5	NULL	NULL	0	NULL	BNP	NULL		bind	NULL				natriuretic peptide receptor A	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_109_13_1680_s_39	15023890	11,12  Studies have established that BNP binds to the natriuretic peptide receptor A, which, via 3'',5''-cGMP, mediates its biological actions.	bind
20158	2	6435	5	NULL	NULL	0	NULL	statement 1	NULL		mediates	NULL				actions of BNP	NULL	biological			NULL		NULL	NULL	NULL	NULL	gw70_circulation_109_13_1680_s_39	15023890	11,12  Studies have established that BNP binds to the natriuretic peptide receptor A, which, via 3'',5''-cGMP, mediates its biological actions.	bind
20159	3	6435	5	NULL	NULL	0	NULL	statement 2	NULL		via	NULL				3'',5''-cGMP	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_109_13_1680_s_39	15023890	11,12  Studies have established that BNP binds to the natriuretic peptide receptor A, which, via 3'',5''-cGMP, mediates its biological actions.	bind
23369	1	6435	7	NULL	NULL	NULL	NULL	BNP	GP		binds to					natriuretic peptide receptor A	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_109_13_1680_s_39	15023890	11,12  Studies have established that BNP binds to the natriuretic peptide receptor A, which, via 3'',5''-cGMP, mediates its biological actions.	bind
23370	2	6435	7	NULL	NULL	NULL	NULL	statement 1	Process		mediates					BNP	GP	actions of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_109_13_1680_s_39	15023890	11,12  Studies have established that BNP binds to the natriuretic peptide receptor A, which, via 3'',5''-cGMP, mediates its biological actions.	bind
23371	3	6435	7	NULL	NULL	NULL	NULL	statement 2	Process		occur via					3'',5''-cGMP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulation_109_13_1680_s_39	15023890	11,12  Studies have established that BNP binds to the natriuretic peptide receptor A, which, via 3'',5''-cGMP, mediates its biological actions.	bind
20160	2	6436	5	NULL	NULL	0	NULL	statement 1	NULL	restimulation of	bind	NULL	may			Fas receptors	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_2_387_s_75	11159176	11- 14 On restimulation, membrane-bound Fas-L molecules may bind to Fas receptors, eg, by membrane folding, to trigger the death signaling cascade that causes the apoptotic suicide of the T cell.	bind
20161	3	6436	5	NULL	NULL	0	NULL	statement 2	NULL		occurs by	NULL				membrane folding	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_2_387_s_75	11159176	11- 14 On restimulation, membrane-bound Fas-L molecules may bind to Fas receptors, eg, by membrane folding, to trigger the death signaling cascade that causes the apoptotic suicide of the T cell.	bind
20162	4	6436	5	NULL	NULL	0	NULL	statement 3	NULL		triggers	NULL				death signaling cascade	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_2_387_s_75	11159176	11- 14 On restimulation, membrane-bound Fas-L molecules may bind to Fas receptors, eg, by membrane folding, to trigger the death signaling cascade that causes the apoptotic suicide of the T cell.	bind
20163	5	6436	5	NULL	NULL	0	NULL	death signaling cascade	NULL		causes	NULL				T cell	NULL	apoptosis of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_2_387_s_75	11159176	11- 14 On restimulation, membrane-bound Fas-L molecules may bind to Fas receptors, eg, by membrane folding, to trigger the death signaling cascade that causes the apoptotic suicide of the T cell.	bind
46189	1	6436	5	NULL	NULL	0	NULL	Fas-L molecules	NULL		bind	NULL				membrane	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_2_387_s_75	11159176	11- 14 On restimulation, membrane-bound Fas-L molecules may bind to Fas receptors, eg, by membrane folding, to trigger the death signaling cascade that causes the apoptotic suicide of the T cell.	bind
23372	2	6436	7	NULL	NULL	NULL	NULL	statement 1	Process		bind					Fas receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_2_387_s_75	11159176	11- 14 On restimulation, membrane-bound Fas-L molecules may bind to Fas receptors, eg, by membrane folding, to trigger the death signaling cascade that causes the apoptotic suicide of the T cell.	bind
23373	3	6436	7	NULL	NULL	NULL	NULL	statement 2	Process		occurs upon					restimulation	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_2_387_s_75	11159176	11- 14 On restimulation, membrane-bound Fas-L molecules may bind to Fas receptors, eg, by membrane folding, to trigger the death signaling cascade that causes the apoptotic suicide of the T cell.	bind
23374	4	6436	7	NULL	NULL	NULL	NULL	statement 2	Process		occurs by					membrane folding	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_2_387_s_75	11159176	11- 14 On restimulation, membrane-bound Fas-L molecules may bind to Fas receptors, eg, by membrane folding, to trigger the death signaling cascade that causes the apoptotic suicide of the T cell.	bind
23375	4	6436	7	NULL	NULL	NULL	NULL	statement 2	Process		trigger					death signaling cascade	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_2_387_s_75	11159176	11- 14 On restimulation, membrane-bound Fas-L molecules may bind to Fas receptors, eg, by membrane folding, to trigger the death signaling cascade that causes the apoptotic suicide of the T cell.	bind
23376	5	6436	7	NULL	NULL	NULL	NULL	statement 4	Process		leads to					T cell	Cell	apoptosis of  			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_2_387_s_75	11159176	11- 14 On restimulation, membrane-bound Fas-L molecules may bind to Fas receptors, eg, by membrane folding, to trigger the death signaling cascade that causes the apoptotic suicide of the T cell.	bind
45752	1	6436	7	NULL	NULL	NULL	NULL	Fas-L molecules	GP		bind					membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_2_387_s_75	11159176	11- 14 On restimulation, membrane-bound Fas-L molecules may bind to Fas receptors, eg, by membrane folding, to trigger the death signaling cascade that causes the apoptotic suicide of the T cell.	bind
20164	1	6437	5	NULL	NULL	0	NULL	XPC	NULL		bind	NULL				XPA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_9_7476_s_121	12486030	11-13 and Fig.  3), it is possible that the binding of XPC (or RPA) to XPA may competitively exclude RPA (or XPC) from the complex.	bind
20165	2	6437	5	NULL	NULL	0	NULL	RPA	NULL		bind	NULL				XPA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_9_7476_s_121	12486030	11-13 and Fig.  3), it is possible that the binding of XPC (or RPA) to XPA may competitively exclude RPA (or XPC) from the complex.	bind
20166	3	6437	5	NULL	NULL	0	NULL	statement 1	NULL		exclude	NULL	may;;competitively			RPA	NULL	from the complex			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_7476_s_121	12486030	11-13 and Fig.  3), it is possible that the binding of XPC (or RPA) to XPA may competitively exclude RPA (or XPC) from the complex.	bind
20167	4	6437	5	NULL	NULL	0	NULL	statement 2	NULL		exclude	NULL	may;;competitively			XPC	NULL	from the complex			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_7476_s_121	12486030	11-13 and Fig.  3), it is possible that the binding of XPC (or RPA) to XPA may competitively exclude RPA (or XPC) from the complex.	bind
23377	1	6437	7	NULL	NULL	NULL	NULL	XPC	GP		bind					XPA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_7476_s_121	12486030	11-13 and Fig.  3), it is possible that the binding of XPC (or RPA) to XPA may competitively exclude RPA (or XPC) from the complex.	bind
23378	2	6437	7	NULL	NULL	NULL	NULL	RPA	GP		bind					XPA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_7476_s_121	12486030	11-13 and Fig.  3), it is possible that the binding of XPC (or RPA) to XPA may competitively exclude RPA (or XPC) from the complex.	bind
23379	3	6437	7	NULL	NULL	NULL	NULL	statement 1	Process		exclude		may;;competitively			RPA	GP	from the complex			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_7476_s_121	12486030	11-13 and Fig.  3), it is possible that the binding of XPC (or RPA) to XPA may competitively exclude RPA (or XPC) from the complex.	bind
23380	4	6437	7	NULL	NULL	NULL	NULL	statement 2	Process		exclude		may;;competitively			XPC	GP	from the complex			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_7476_s_121	12486030	11-13 and Fig.  3), it is possible that the binding of XPC (or RPA) to XPA may competitively exclude RPA (or XPC) from the complex.	bind
20168	1	6438	5	NULL	NULL	0	NULL	cadherin-like protein	NULL		bind	NULL				Cry1Aa	NULL				NULL	M. sexta	NULL	NULL	NULL	NULL	gw60_insectbiochemmolbiol_30_11_1069_s_10	10989294	11.2), the exception being a cadherin-like protein which bound Cry1Aa in  M. sexta ( Valdamudi et al., 1995;   Francis and Bulla, 1997;   Keeton and Bulla, 1997).	bind
23381	1	6438	7	NULL	NULL	NULL	NULL	 cadherin-like protein	GP		bind					Cry1Aa	GP				NULL	M. sexta	NULL	NULL	NULL	NULL	gw60_insectbiochemmolbiol_30_11_1069_s_10	10989294	11.2), the exception being a cadherin-like protein which bound Cry1Aa in  M. sexta ( Valdamudi et al., 1995;   Francis and Bulla, 1997;   Keeton and Bulla, 1997).	bind
20169	1	6440	5	NULL	NULL	0	NULL	Ag+	NULL		bind	NULL				metallothionein	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochemistry_35_44_8909290_s_1	8909290	111Cd NMR studies of the domain specificity of Ag+ and Cu+ binding to metallothionein..	bind
20170	2	6440	5	NULL	NULL	0	NULL	Cu+	NULL		bind	NULL				metallothionein	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochemistry_35_44_8909290_s_1	8909290	111Cd NMR studies of the domain specificity of Ag+ and Cu+ binding to metallothionein..	bind
23382	1	6440	7	NULL	NULL	NULL	NULL	Ag+	Chemical		bind					metallothionein	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_biochemistry_35_44_8909290_s_1	8909290	111Cd NMR studies of the domain specificity of Ag+ and Cu+ binding to metallothionein..	bind
23383	2	6440	7	NULL	NULL	NULL	NULL	Cu+	Chemical		bind					metallothionein	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_biochemistry_35_44_8909290_s_1	8909290	111Cd NMR studies of the domain specificity of Ag+ and Cu+ binding to metallothionein..	bind
20171	1	6441	5	NULL	NULL	0	NULL	ERalpha	NULL		bind	NULL	constitutively			PI3K	NULL		p85alpha subunit		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_123	12482819	113 Interestingly, ERalpha binds constitutively to the p85alpha subunit of PI3K and activates PI3K/Akt in an E2-independent manner, implicating a feed-forward mechanism of ERalpha activation.	bind
20172	2	6441	5	10	NULL	0	NULL	statement 1			activates					PI3K/Akt					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_123	12482819	113 Interestingly, ERalpha binds constitutively to the p85alpha subunit of PI3K and activates PI3K/Akt in an E2-independent manner, implicating a feed-forward mechanism of ERalpha activation.	bind
20173	3	6441	5	NULL	NULL	0	NULL	statement 2	NULL		is independent of	NULL				E2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_123	12482819	113 Interestingly, ERalpha binds constitutively to the p85alpha subunit of PI3K and activates PI3K/Akt in an E2-independent manner, implicating a feed-forward mechanism of ERalpha activation.	bind
20174	4	6441	5	NULL	NULL	0	NULL	statement 3	NULL		implicate	NULL				feed-forward mechanism of ERalpha	NULL	activation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_123	12482819	113 Interestingly, ERalpha binds constitutively to the p85alpha subunit of PI3K and activates PI3K/Akt in an E2-independent manner, implicating a feed-forward mechanism of ERalpha activation.	bind
23384	1	6441	7	NULL	NULL	NULL	NULL	ERalpha	GP		binds		constitutively			PI3K	GP		p85alpha subunit		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_123	12482819	113 Interestingly, ERalpha binds constitutively to the p85alpha subunit of PI3K and activates PI3K/Akt in an E2-independent manner, implicating a feed-forward mechanism of ERalpha activation.	bind
23385	2	6441	7	NULL	NULL	NULL	NULL	statement 1	Process		activates					PI3K/Akt	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_123	12482819	113 Interestingly, ERalpha binds constitutively to the p85alpha subunit of PI3K and activates PI3K/Akt in an E2-independent manner, implicating a feed-forward mechanism of ERalpha activation.	bind
23386	3	6441	7	NULL	NULL	NULL	NULL	statement 2	Process		is independent of					E2	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_123	12482819	113 Interestingly, ERalpha binds constitutively to the p85alpha subunit of PI3K and activates PI3K/Akt in an E2-independent manner, implicating a feed-forward mechanism of ERalpha activation.	bind
23387	4	6441	7	NULL	NULL	NULL	NULL	statement 2	Process		implicate					feed-forward mechanism ofER alpha	Process	activation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_123	12482819	113 Interestingly, ERalpha binds constitutively to the p85alpha subunit of PI3K and activates PI3K/Akt in an E2-independent manner, implicating a feed-forward mechanism of ERalpha activation.	bind
20175	1	6442	5	NULL	NULL	0	NULL	Cd(II)	NULL		bind	NULL				Suwannee River fulvic acid	NULL				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_ann-chim_95_7-8_16235791_s_1	16235791	113Cd NMR and fluorescence studies of multiple binding mechanisms of Cd(II) by the Suwannee River fulvic acid..	bind
23388	1	6442	7	NULL	NULL	NULL	NULL	Cd(II) 	Chemical		bind					Suwannee River fulvic acid	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_ann-chim_95_7-8_16235791_s_1	16235791	113Cd NMR and fluorescence studies of multiple binding mechanisms of Cd(II) by the Suwannee River fulvic acid..	bind
20176	1	6443	5	NULL	NULL	0	NULL		NULL	prebending	destabilizes	NULL			estrogen response element	estrogen receptor	NULL	binding of	DNA binding domain		NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_656	11452016	114       Kim,J., DeHaan,G., Nardulli,A.M. and Shapiro,D.J. (1997) Prebending the estrogen response element destabilized binding of the estrogen receptor DNA binding domain.	bind
23389	1	6443	7	NULL	NULL	NULL	NULL			Prebending	destabilize				estrogen response element	estrogen receptor 	GP	binding of	DNA binding domain		NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_656	11452016	114       Kim,J., DeHaan,G., Nardulli,A.M. and Shapiro,D.J. (1997) Prebending the estrogen response element destabilized binding of the estrogen receptor DNA binding domain.	bind
23126	1	6444	5	10	NULL	0	NULL	1178T			bind		dramatically reduced			PI 3-kinase					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_49_29286_s_122	7493960	1178T ( 31) shows dramatically reduced binding  of PI 3-kinase, while Y250F ( 8,  9,  32) is  deficient in associating with SHC and thereby unable to initiate  signaling through Ras. NG59 ( 38) binds none of the molecules  characterized so far, 1387T (a truncated mutant protein lacking the  membrane anchor sequence) only binds PP2A( 39,  60) ,  and dl1015 associates with all cellular enzymes described so far, but  is unable to activate PI 3-kinase( 40,  41) .	bind
23127	2	6444	5	NULL	NULL	0	NULL		NULL		is deficient in associating with	NULL		Y250F		SHC	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_49_29286_s_122	7493960	1178T ( 31) shows dramatically reduced binding  of PI 3-kinase, while Y250F ( 8,  9,  32) is  deficient in associating with SHC and thereby unable to initiate  signaling through Ras. NG59 ( 38) binds none of the molecules  characterized so far, 1387T (a truncated mutant protein lacking the  membrane anchor sequence) only binds PP2A( 39,  60) ,  and dl1015 associates with all cellular enzymes described so far, but  is unable to activate PI 3-kinase( 40,  41) .	bind
23128	3	6444	5	10	NULL	0	NULL	statement 2	NULL		does not initiate	NULL				Ras	NULL	signaling through			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_49_29286_s_122	7493960	1178T ( 31) shows dramatically reduced binding  of PI 3-kinase, while Y250F ( 8,  9,  32) is  deficient in associating with SHC and thereby unable to initiate  signaling through Ras. NG59 ( 38) binds none of the molecules  characterized so far, 1387T (a truncated mutant protein lacking the  membrane anchor sequence) only binds PP2A( 39,  60) ,  and dl1015 associates with all cellular enzymes described so far, but  is unable to activate PI 3-kinase( 40,  41) .	bind
23129	4	6444	5	NULL	NULL	0	NULL	1387T	NULL		is	NULL				truncated mutant protein lacking the membrane anchor sequence	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_49_29286_s_122	7493960	1178T ( 31) shows dramatically reduced binding  of PI 3-kinase, while Y250F ( 8,  9,  32) is  deficient in associating with SHC and thereby unable to initiate  signaling through Ras. NG59 ( 38) binds none of the molecules  characterized so far, 1387T (a truncated mutant protein lacking the  membrane anchor sequence) only binds PP2A( 39,  60) ,  and dl1015 associates with all cellular enzymes described so far, but  is unable to activate PI 3-kinase( 40,  41) .	bind
23130	5	6444	5	NULL	NULL	0	NULL	1387T	NULL		bind	NULL	only			PP2A	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_49_29286_s_122	7493960	1178T ( 31) shows dramatically reduced binding  of PI 3-kinase, while Y250F ( 8,  9,  32) is  deficient in associating with SHC and thereby unable to initiate  signaling through Ras. NG59 ( 38) binds none of the molecules  characterized so far, 1387T (a truncated mutant protein lacking the  membrane anchor sequence) only binds PP2A( 39,  60) ,  and dl1015 associates with all cellular enzymes described so far, but  is unable to activate PI 3-kinase( 40,  41) .	bind
23131	6	6444	5	NULL	NULL	0	NULL	dl1015 	NULL		associates with	NULL				cellular enzymes	NULL	all			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_49_29286_s_122	7493960	1178T ( 31) shows dramatically reduced binding  of PI 3-kinase, while Y250F ( 8,  9,  32) is  deficient in associating with SHC and thereby unable to initiate  signaling through Ras. NG59 ( 38) binds none of the molecules  characterized so far, 1387T (a truncated mutant protein lacking the  membrane anchor sequence) only binds PP2A( 39,  60) ,  and dl1015 associates with all cellular enzymes described so far, but  is unable to activate PI 3-kinase( 40,  41) .	bind
23132	7	6444	5	NULL	NULL	0	NULL	dl1015	NULL		does not activate	NULL				PI 3-kinase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_49_29286_s_122	7493960	1178T ( 31) shows dramatically reduced binding  of PI 3-kinase, while Y250F ( 8,  9,  32) is  deficient in associating with SHC and thereby unable to initiate  signaling through Ras. NG59 ( 38) binds none of the molecules  characterized so far, 1387T (a truncated mutant protein lacking the  membrane anchor sequence) only binds PP2A( 39,  60) ,  and dl1015 associates with all cellular enzymes described so far, but  is unable to activate PI 3-kinase( 40,  41) .	bind
23133	8	6444	5	NULL	NULL	0	NULL	NG59	NULL		does not bind	NULL				characterized molecules	NULL	any			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_49_29286_s_122	7493960	1178T ( 31) shows dramatically reduced binding  of PI 3-kinase, while Y250F ( 8,  9,  32) is  deficient in associating with SHC and thereby unable to initiate  signaling through Ras. NG59 ( 38) binds none of the molecules  characterized so far, 1387T (a truncated mutant protein lacking the  membrane anchor sequence) only binds PP2A( 39,  60) ,  and dl1015 associates with all cellular enzymes described so far, but  is unable to activate PI 3-kinase( 40,  41) .	bind
23456	1	6444	7	NULL	NULL	NULL	NULL	1178T	NucleicAcid		bind		reduced			PI 3-kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_49_29286_s_122	7493960	1178T ( 31) shows dramatically reduced binding  of PI 3-kinase, while Y250F ( 8,  9,  32) is  deficient in associating with SHC and thereby unable to initiate  signaling through Ras. NG59 ( 38) binds none of the molecules  characterized so far, 1387T (a truncated mutant protein lacking the  membrane anchor sequence) only binds PP2A( 39,  60) ,  and dl1015 associates with all cellular enzymes described so far, but  is unable to activate PI 3-kinase( 40,  41) .	bind
23457	2	6444	7	NULL	NULL	NULL	NULL				is defecient in			Y250F		SHC	GP	associating with			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_49_29286_s_122	7493960	1178T ( 31) shows dramatically reduced binding  of PI 3-kinase, while Y250F ( 8,  9,  32) is  deficient in associating with SHC and thereby unable to initiate  signaling through Ras. NG59 ( 38) binds none of the molecules  characterized so far, 1387T (a truncated mutant protein lacking the  membrane anchor sequence) only binds PP2A( 39,  60) ,  and dl1015 associates with all cellular enzymes described so far, but  is unable to activate PI 3-kinase( 40,  41) .	bind
23458	3	6444	7	NULL	NULL	NULL	NULL	statement 2	Process		is unable to 					Ras	GP	initiate signaling through			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_49_29286_s_122	7493960	1178T ( 31) shows dramatically reduced binding  of PI 3-kinase, while Y250F ( 8,  9,  32) is  deficient in associating with SHC and thereby unable to initiate  signaling through Ras. NG59 ( 38) binds none of the molecules  characterized so far, 1387T (a truncated mutant protein lacking the  membrane anchor sequence) only binds PP2A( 39,  60) ,  and dl1015 associates with all cellular enzymes described so far, but  is unable to activate PI 3-kinase( 40,  41) .	bind
23459	4	6444	7	NULL	NULL	NULL	NULL	1387T	GP		binds					PP2A	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_49_29286_s_122	7493960	1178T ( 31) shows dramatically reduced binding  of PI 3-kinase, while Y250F ( 8,  9,  32) is  deficient in associating with SHC and thereby unable to initiate  signaling through Ras. NG59 ( 38) binds none of the molecules  characterized so far, 1387T (a truncated mutant protein lacking the  membrane anchor sequence) only binds PP2A( 39,  60) ,  and dl1015 associates with all cellular enzymes described so far, but  is unable to activate PI 3-kinase( 40,  41) .	bind
23460	5	6444	7	NULL	NULL	NULL	NULL	dl1015	NucleicAcid		associate with					cellular enzymes	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_49_29286_s_122	7493960	1178T ( 31) shows dramatically reduced binding  of PI 3-kinase, while Y250F ( 8,  9,  32) is  deficient in associating with SHC and thereby unable to initiate  signaling through Ras. NG59 ( 38) binds none of the molecules  characterized so far, 1387T (a truncated mutant protein lacking the  membrane anchor sequence) only binds PP2A( 39,  60) ,  and dl1015 associates with all cellular enzymes described so far, but  is unable to activate PI 3-kinase( 40,  41) .	bind
23461	6	6444	7	NULL	NULL	NULL	NULL	dl1015	NucleicAcid		is unable to activate					PI 3-kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_49_29286_s_122	7493960	1178T ( 31) shows dramatically reduced binding  of PI 3-kinase, while Y250F ( 8,  9,  32) is  deficient in associating with SHC and thereby unable to initiate  signaling through Ras. NG59 ( 38) binds none of the molecules  characterized so far, 1387T (a truncated mutant protein lacking the  membrane anchor sequence) only binds PP2A( 39,  60) ,  and dl1015 associates with all cellular enzymes described so far, but  is unable to activate PI 3-kinase( 40,  41) .	bind
23462	7	6444	7	NULL	NULL	NULL	NULL	1387T	GP		is a type of					truncated mutant protein lacking the membrane anchor sequence	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_49_29286_s_122	7493960	1178T ( 31) shows dramatically reduced binding  of PI 3-kinase, while Y250F ( 8,  9,  32) is  deficient in associating with SHC and thereby unable to initiate  signaling through Ras. NG59 ( 38) binds none of the molecules  characterized so far, 1387T (a truncated mutant protein lacking the  membrane anchor sequence) only binds PP2A( 39,  60) ,  and dl1015 associates with all cellular enzymes described so far, but  is unable to activate PI 3-kinase( 40,  41) .	bind
23108	1	6446	5	NULL	NULL	0	NULL	11F8	NULL		forms a complex with	NULL				histone	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
23109	2	6446	5	NULL	NULL	0	NULL	9F11	NULL		forms a complex with	NULL				histone	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
23110	3	6446	5	NULL	NULL	0	NULL	11F8	NULL		forms a complex with	NULL				ssDNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
23111	4	6446	5	NULL	NULL	0	NULL	9F11	NULL		forms a complex with	NULL				ssDNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
23112	5	6446	5	NULL	NULL	0	NULL	poly(dT)	NULL		bind	NULL				laminin	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
23113	6	6446	5	NULL	NULL	0	NULL	poly(dT)	NULL		bind	NULL				collagen IV	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
23116	7	6446	5	NULL	NULL	0	NULL	poly(dT)	NULL		does not bind	NULL				heparan sulfate	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
23117	8	6446	5	NULL	NULL	0	NULL	poly(dT)	NULL		does not bind	NULL				fibronectin	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
23118	9	6446	5	NULL	NULL	0	NULL	11F8	NULL		forms a complex with	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
23119	10	6446	5	NULL	NULL	0	NULL	11F8	NULL		forms a complex with	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
23120	11	6446	5	NULL	NULL	0	NULL	9F11	NULL		forms a complex with	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
23121	12	6446	5	NULL	NULL	0	NULL	9F11	NULL		forms a complex with	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
23122	13	6446	5	NULL	NULL	0	NULL	statement 3	NULL		is an alternative to	NULL				statement 9	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
23123	14	6446	5	NULL	NULL	0	NULL	statement 3	NULL		is an alternative to	NULL				statement 10	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
23124	15	6446	5	NULL	NULL	0	NULL	statement 4	NULL		is an alternative to	NULL				statement 11	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
23125	16	6446	5	NULL	NULL	0	NULL	statement 4	NULL		is an alternative to	NULL				statement 12	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
23463	1	6446	7	NULL	NULL	NULL	NULL	11F8	NucleicAcid		complex with					histone	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
23464	2	6446	7	NULL	NULL	NULL	NULL	 9F11	NucleicAcid		complex with					histone	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
23465	3	6446	7	NULL	NULL	NULL	NULL	11F8	NucleicAcid		complex with					ssDNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
23466	4	6446	7	NULL	NULL	NULL	NULL	9F11	NucleicAcid		complex with					ssDNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
23467	5	6446	7	NULL	NULL	NULL	NULL	11F8	NucleicAcid		complex with					poly(dT)	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
23468	6	6446	7	NULL	NULL	NULL	NULL	9F11	NucleicAcid		complex with					poly(dT)	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
23469	7	6446	7	NULL	NULL	NULL	NULL	statement 1	Process		is simultaneously with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
23470	8	6446	7	NULL	NULL	NULL	NULL	statement 2	Process		is simultaneously with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
23471	9	6446	7	NULL	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
23472	10	6446	7	NULL	NULL	NULL	NULL	statement 4	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
23473	11	6446	7	NULL	NULL	NULL	NULL	statement 1	Process		binds to					laminin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
24391	12	6446	7	NULL	NULL	NULL	NULL	statement 2	Process		binds to					laminin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
24392	13	6446	7	NULL	NULL	NULL	NULL	statement 1	Process		binds to					collagen IV	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
24393	14	6446	7	NULL	NULL	NULL	NULL	statement 2	Process		binds to					collagen IV	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
24394	15	6446	7	NULL	NULL	NULL	NULL	statement 1	Process		does not bind					heparan sulfate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
24395	16	6446	7	NULL	NULL	NULL	NULL	statement 2	Process		does not bind					heparan sulfate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
24396	17	6446	7	NULL	NULL	NULL	NULL	statement 1	Process		does not bind					fibronectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
24397	18	6446	7	NULL	NULL	NULL	NULL	statement 2	Process		does not bind					fibronectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_7_1748_s_202	8601641	11F8 and 9F11 both form complexes with histone and either ssDNA or poly(dT) that bind to laminin and collagen IV,  but not to heparan sulfate or fibronectin.	bind
20177	1	6447	5	10	NULL	0	NULL	spermine			bind					Z-DNA				d(m5CGm5CGm5CG)2	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_419_s_377	11788703	12       Banville,D.L., Feuerstein,B.G. and Shafer,R.H. (1991) 1H and 31P nuclear magnetic resonance studies of spermine binding to the Z-DNA form of d(m5CGm5CGm5CG)2: evidence for decreased spermine mobility.	bind
20178	2	6447	5	NULL	NULL	0	NULL	statement 1	NULL		is an evidence for	NULL				spermine	NULL	decreased mobility of			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_419_s_377	11788703	12       Banville,D.L., Feuerstein,B.G. and Shafer,R.H. (1991) 1H and 31P nuclear magnetic resonance studies of spermine binding to the Z-DNA form of d(m5CGm5CGm5CG)2: evidence for decreased spermine mobility.	bind
23474	1	6447	7	NULL	NULL	NULL	NULL	spermine	GP		binds to					 Z-DNA	NucleicAcid			d(m5CGm5CGm5CG)2	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_419_s_377	11788703	12       Banville,D.L., Feuerstein,B.G. and Shafer,R.H. (1991) 1H and 31P nuclear magnetic resonance studies of spermine binding to the Z-DNA form of d(m5CGm5CGm5CG)2: evidence for decreased spermine mobility.	bind
20180	1	6450	5	NULL	NULL	0	NULL	TnI	NULL		moves away from	NULL				actin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_1_9_s_24	null	12  13  The calcium-dependent movement of TnI away from actin reveals a tropomyosin binding site, which results in movement of tropomyosin away from high-affinity myosin binding sites on actin.	bind
20181	3	6450	5	NULL	NULL	0	NULL	statement 1	NULL		reveals	NULL					NULL		tropomyosin binding site		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_1_9_s_24	null	12  13  The calcium-dependent movement of TnI away from actin reveals a tropomyosin binding site, which results in movement of tropomyosin away from high-affinity myosin binding sites on actin.	bind
20182	4	6450	5	NULL	NULL	0	NULL	tropomyosin	NULL		moves away from	NULL				actin	NULL	 high-affinity	myosin binding sites		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_1_9_s_24	null	12  13  The calcium-dependent movement of TnI away from actin reveals a tropomyosin binding site, which results in movement of tropomyosin away from high-affinity myosin binding sites on actin.	bind
20183	5	6450	5	NULL	NULL	0	NULL	statement 3	NULL		results in	NULL				statement 4	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_1_9_s_24	null	12  13  The calcium-dependent movement of TnI away from actin reveals a tropomyosin binding site, which results in movement of tropomyosin away from high-affinity myosin binding sites on actin.	bind
30030	2	6450	5	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				calcium	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_1_9_s_24	null	12  13  The calcium-dependent movement of TnI away from actin reveals a tropomyosin binding site, which results in movement of tropomyosin away from high-affinity myosin binding sites on actin.	bind
23605	1	6450	7	NULL	NULL	NULL	NULL	TnI 	GP		move away from					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_1_9_s_24	null	12  13  The calcium-dependent movement of TnI away from actin reveals a tropomyosin binding site, which results in movement of tropomyosin away from high-affinity myosin binding sites on actin.	bind
23606	2	6450	7	NULL	NULL	NULL	NULL	statement 1	Process		is dependent on					calcium	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_1_9_s_24	null	12  13  The calcium-dependent movement of TnI away from actin reveals a tropomyosin binding site, which results in movement of tropomyosin away from high-affinity myosin binding sites on actin.	bind
23607	3	6450	7	NULL	NULL	NULL	NULL	statement 1	Process		reveals								tropomyosin binding site		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_1_9_s_24	null	12  13  The calcium-dependent movement of TnI away from actin reveals a tropomyosin binding site, which results in movement of tropomyosin away from high-affinity myosin binding sites on actin.	bind
23608	4	6450	7	NULL	NULL	NULL	NULL	tropomyosin	GP		move away from					actin	GP	high-affinity	myosin binding site		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_1_9_s_24	null	12  13  The calcium-dependent movement of TnI away from actin reveals a tropomyosin binding site, which results in movement of tropomyosin away from high-affinity myosin binding sites on actin.	bind
23609	5	6450	7	NULL	NULL	NULL	NULL	statement 3	Process		results in					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_1_9_s_24	null	12  13  The calcium-dependent movement of TnI away from actin reveals a tropomyosin binding site, which results in movement of tropomyosin away from high-affinity myosin binding sites on actin.	bind
20184	1	6451	5	NULL	NULL	0	NULL	tryp-VLDL	NULL		does not bind	NULL				LDL receptors	NULL	partially purified bovine			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_968_s_45	9633939	12  13 27  Functional loss of apoE was demonstrated by lack of binding of tryp-VLDL to partially purified bovine LDL receptors on ligand blots.	bind
20185	2	6451	5	NULL	NULL	0	NULL	statement 1	NULL		demonstrate	NULL				apoE	NULL	functional loss of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_968_s_45	9633939	12  13 27  Functional loss of apoE was demonstrated by lack of binding of tryp-VLDL to partially purified bovine LDL receptors on ligand blots.	bind
23610	1	6451	7	NULL	NULL	NULL	NULL	tryp-VLDL	GP		does not bind					LDL receptors	GP	partially purified bovine			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_968_s_45	9633939	12  13 27  Functional loss of apoE was demonstrated by lack of binding of tryp-VLDL to partially purified bovine LDL receptors on ligand blots.	bind
23611	2	6451	7	NULL	NULL	NULL	NULL	apoE	GP	functional loss of	demonstrate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_968_s_45	9633939	12  13 27  Functional loss of apoE was demonstrated by lack of binding of tryp-VLDL to partially purified bovine LDL receptors on ligand blots.	bind
20186	1	6452	5	NULL	NULL	0	NULL	vWF multimers	NULL	large	is adsorbed onto	NULL				collagen I 	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_91_5_1354_s_28	7867173	12  Adhesion at elevated shear rates in our system is the result of the adsorption of large vWF multimers onto collagen I and the binding of platelet GPIb to the insolubilized vWF.	bind
20187	2	6452	5	10	NULL	0	NULL	GPIb		platelet	bind					vWF		insolubilized			NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1354_s_28	7867173	12  Adhesion at elevated shear rates in our system is the result of the adsorption of large vWF multimers onto collagen I and the binding of platelet GPIb to the insolubilized vWF.	bind
20188	3	6452	5	NULL	NULL	0	NULL	statement 1	NULL		results in	NULL				adhesion	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1354_s_28	7867173	12  Adhesion at elevated shear rates in our system is the result of the adsorption of large vWF multimers onto collagen I and the binding of platelet GPIb to the insolubilized vWF.	bind
20189	4	6452	5	NULL	NULL	0	NULL	statement 2	NULL		results in	NULL				adhesion	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1354_s_28	7867173	12  Adhesion at elevated shear rates in our system is the result of the adsorption of large vWF multimers onto collagen I and the binding of platelet GPIb to the insolubilized vWF.	bind
30031	5	6452	5	NULL	NULL	0	NULL	statement 3	NULL		occurs at	NULL				shear rates	NULL	elevated			NULL		0	NULL	NULL	NULL	gw60_circulation_91_5_1354_s_28	7867173	12  Adhesion at elevated shear rates in our system is the result of the adsorption of large vWF multimers onto collagen I and the binding of platelet GPIb to the insolubilized vWF.	bind
30032	6	6452	5	NULL	NULL	0	NULL	statement 4	NULL		occurs at	NULL				shear rates	NULL	elevated			NULL		0	NULL	NULL	NULL	gw60_circulation_91_5_1354_s_28	7867173	12  Adhesion at elevated shear rates in our system is the result of the adsorption of large vWF multimers onto collagen I and the binding of platelet GPIb to the insolubilized vWF.	bind
23612	1	6452	7	NULL	NULL	NULL	NULL	vWF multimers	GP	large	adsorb to					collagen I	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1354_s_28	7867173	12  Adhesion at elevated shear rates in our system is the result of the adsorption of large vWF multimers onto collagen I and the binding of platelet GPIb to the insolubilized vWF.	bind
23613	2	6452	7	NULL	NULL	NULL	NULL	GPIb	GP	platelet	bind					vWF	GP	insolubilized			NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1354_s_28	7867173	12  Adhesion at elevated shear rates in our system is the result of the adsorption of large vWF multimers onto collagen I and the binding of platelet GPIb to the insolubilized vWF.	bind
30844	3	6452	7	NULL	NULL	NULL	NULL	statement 1	Process		results in					adhesion	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1354_s_28	7867173	12  Adhesion at elevated shear rates in our system is the result of the adsorption of large vWF multimers onto collagen I and the binding of platelet GPIb to the insolubilized vWF.	bind
30845	4	6452	7	NULL	NULL	NULL	NULL	statement 2	Process		results in					adhesion	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1354_s_28	7867173	12  Adhesion at elevated shear rates in our system is the result of the adsorption of large vWF multimers onto collagen I and the binding of platelet GPIb to the insolubilized vWF.	bind
30846	5	6452	7	NULL	NULL	NULL	NULL	statement 3	Process		occurs at					shear rates	Process	elevated			NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1354_s_28	7867173	12  Adhesion at elevated shear rates in our system is the result of the adsorption of large vWF multimers onto collagen I and the binding of platelet GPIb to the insolubilized vWF.	bind
30847	6	6452	7	NULL	NULL	NULL	NULL	statement 4	Process		occurs at					shear rates	Process	elevated			NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1354_s_28	7867173	12  Adhesion at elevated shear rates in our system is the result of the adsorption of large vWF multimers onto collagen I and the binding of platelet GPIb to the insolubilized vWF.	bind
20190	1	6454	5	10	NULL	0	NULL	thrombomodulin	NULL		bind	NULL				thrombin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_12_1118_s_167	10082479	12  Another downregulated gene was thrombomodulin (-2.6-fold at 24 hours), an integral membrane glycoprotein that binds thrombin, the final enzyme of the procoagulant pathway 31 ; we confirmed by Northern analysis that thrombomodulin was downregulated 3.3 plus-or-minus 1.0-fold by cyclic deformation (Figure 6  ).	bind
20191	2	6454	5	10	NULL	0	NULL	thrombin			is final enzyme of					procoagulant pathway					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_12_1118_s_167	10082479	12  Another downregulated gene was thrombomodulin (-2.6-fold at 24 hours), an integral membrane glycoprotein that binds thrombin, the final enzyme of the procoagulant pathway 31 ; we confirmed by Northern analysis that thrombomodulin was downregulated 3.3 plus-or-minus 1.0-fold by cyclic deformation (Figure 6  ).	bind
20192	3	6454	5	NULL	NULL	0	NULL	thrombomodulin	NULL		is downregulated by	NULL				cyclic deformation	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_85_12_1118_s_167	10082479	12  Another downregulated gene was thrombomodulin (-2.6-fold at 24 hours), an integral membrane glycoprotein that binds thrombin, the final enzyme of the procoagulant pathway 31 ; we confirmed by Northern analysis that thrombomodulin was downregulated 3.3 plus-or-minus 1.0-fold by cyclic deformation (Figure 6  ).	bind
45619	4	6454	5	10	NULL	0	NULL	thrombomodulin	NULL		is a type of	NULL				integral membrane glycoprotein	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_85_12_1118_s_167	10082479	12  Another downregulated gene was thrombomodulin (-2.6-fold at 24 hours), an integral membrane glycoprotein that binds thrombin, the final enzyme of the procoagulant pathway 31 ; we confirmed by Northern analysis that thrombomodulin was downregulated 3.3 plus-or-minus 1.0-fold by cyclic deformation (Figure 6  ).	bind
23614	1	6454	7	NULL	NULL	NULL	NULL	thrombomodulin	GP		binds					thrombin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_12_1118_s_167	10082479	12  Another downregulated gene was thrombomodulin (-2.6-fold at 24 hours), an integral membrane glycoprotein that binds thrombin, the final enzyme of the procoagulant pathway 31 ; we confirmed by Northern analysis that thrombomodulin was downregulated 3.3 plus-or-minus 1.0-fold by cyclic deformation (Figure 6  ).	bind
23615	2	6454	7	NULL	NULL	NULL	NULL	thrombin	GP		is the final enzyme of					procoagulant pathway	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_12_1118_s_167	10082479	12  Another downregulated gene was thrombomodulin (-2.6-fold at 24 hours), an integral membrane glycoprotein that binds thrombin, the final enzyme of the procoagulant pathway 31 ; we confirmed by Northern analysis that thrombomodulin was downregulated 3.3 plus-or-minus 1.0-fold by cyclic deformation (Figure 6  ).	bind
23616	3	6454	7	NULL	NULL	NULL	NULL	cyclic deformation 	Process		downregulates					thrombomodulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_12_1118_s_167	10082479	12  Another downregulated gene was thrombomodulin (-2.6-fold at 24 hours), an integral membrane glycoprotein that binds thrombin, the final enzyme of the procoagulant pathway 31 ; we confirmed by Northern analysis that thrombomodulin was downregulated 3.3 plus-or-minus 1.0-fold by cyclic deformation (Figure 6  ).	bind
45620	4	6454	7	NULL	NULL	NULL	NULL	thrombomodulin	GP		is a type of					integral membrane glycoprotein	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_12_1118_s_167	10082479	12  Another downregulated gene was thrombomodulin (-2.6-fold at 24 hours), an integral membrane glycoprotein that binds thrombin, the final enzyme of the procoagulant pathway 31 ; we confirmed by Northern analysis that thrombomodulin was downregulated 3.3 plus-or-minus 1.0-fold by cyclic deformation (Figure 6  ).	bind
20193	1	6455	5	NULL	NULL	0	NULL	VLDL particles	NULL		bind	NULL				LDL receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_5_1354_s_100	10323790	12  As both VLDL and LDL particles bind to the LDL receptor, whereas only VLDL enhances PAI-1 secretion from endothelial and liver cells in culture, the TG content of the lipoprotein particle might be important for the induction of PAI-1.	bind
20194	2	6455	5	NULL	NULL	0	NULL	LDL particles	NULL		bind	NULL				LDL receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_5_1354_s_100	10323790	12  As both VLDL and LDL particles bind to the LDL receptor, whereas only VLDL enhances PAI-1 secretion from endothelial and liver cells in culture, the TG content of the lipoprotein particle might be important for the induction of PAI-1.	bind
20195	3	6455	5	NULL	NULL	0	NULL	VLDL	NULL		enhances	NULL	only			PAI-1	NULL	secretion of			NULL	from endothelial cells in culture	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_5_1354_s_100	10323790	12  As both VLDL and LDL particles bind to the LDL receptor, whereas only VLDL enhances PAI-1 secretion from endothelial and liver cells in culture, the TG content of the lipoprotein particle might be important for the induction of PAI-1.	bind
20196	4	6455	5	NULL	NULL	0	NULL	VLDL	NULL		enhances	NULL	only			PAI-1	NULL	secretion of			NULL	from liver cells in culture	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_5_1354_s_100	10323790	12  As both VLDL and LDL particles bind to the LDL receptor, whereas only VLDL enhances PAI-1 secretion from endothelial and liver cells in culture, the TG content of the lipoprotein particle might be important for the induction of PAI-1.	bind
20197	5	6455	5	NULL	NULL	0	NULL	lipoprotein particle	NULL	TG content of	is important for	NULL	might be			PAI-1	NULL	induction of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_5_1354_s_100	10323790	12  As both VLDL and LDL particles bind to the LDL receptor, whereas only VLDL enhances PAI-1 secretion from endothelial and liver cells in culture, the TG content of the lipoprotein particle might be important for the induction of PAI-1.	bind
23617	1	6455	7	NULL	NULL	NULL	NULL	VLDL particles	GP		bind					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_5_1354_s_100	10323790	12  As both VLDL and LDL particles bind to the LDL receptor, whereas only VLDL enhances PAI-1 secretion from endothelial and liver cells in culture, the TG content of the lipoprotein particle might be important for the induction of PAI-1.	bind
23618	2	6455	7	NULL	NULL	NULL	NULL	LDL particles	GP		bind					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_5_1354_s_100	10323790	12  As both VLDL and LDL particles bind to the LDL receptor, whereas only VLDL enhances PAI-1 secretion from endothelial and liver cells in culture, the TG content of the lipoprotein particle might be important for the induction of PAI-1.	bind
23619	3	6455	7	NULL	NULL	NULL	NULL	VLDL	GP		enhance					PAI-1	GP	secretion of			NULL	from endothelial cells in culture	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_5_1354_s_100	10323790	12  As both VLDL and LDL particles bind to the LDL receptor, whereas only VLDL enhances PAI-1 secretion from endothelial and liver cells in culture, the TG content of the lipoprotein particle might be important for the induction of PAI-1.	bind
23620	4	6455	7	NULL	NULL	NULL	NULL	VLDL	GP		enhance					PAI-1	GP	secretion of			NULL	liver cells in culture	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_5_1354_s_100	10323790	12  As both VLDL and LDL particles bind to the LDL receptor, whereas only VLDL enhances PAI-1 secretion from endothelial and liver cells in culture, the TG content of the lipoprotein particle might be important for the induction of PAI-1.	bind
23621	5	6455	7	NULL	NULL	NULL	NULL	lipoprotein 	GP	TG content of	is important for					PAI-1	GP	induction of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_5_1354_s_100	10323790	12  As both VLDL and LDL particles bind to the LDL receptor, whereas only VLDL enhances PAI-1 secretion from endothelial and liver cells in culture, the TG content of the lipoprotein particle might be important for the induction of PAI-1.	bind
20198	1	6456	5	NULL	NULL	0	NULL	p60c-Src	NULL		bind	NULL	weakly			Fak	NULL				NULL	in the myocardium of control rats	NULL	NULL	NULL	NULL	gw60_circulationres_87_7_558_s_95	11009560	12  Coimmunoprecipitation assays with anti-Fak and anti - c-Src antibodies showed only a weak binding of p60c-Src to Fak in the myocardium of control rats (Figure 4A  ).	bind
23623	1	6456	7	NULL	NULL	NULL	NULL	p60c-Src	GP		bind		weakly			Fak	GP				NULL	myocardium of control rats	NULL	NULL	NULL	NULL	gw60_circulationres_87_7_558_s_95	11009560	12  Coimmunoprecipitation assays with anti-Fak and anti - c-Src antibodies showed only a weak binding of p60c-Src to Fak in the myocardium of control rats (Figure 4A  ).	bind
20199	1	6457	5	NULL	NULL	0	NULL	CRP	NULL		is found within	NULL				endothelial vessel walls	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_97_5_425_s_78	9490235	12  Experimental work also suggests that CRP can be found within endothelial vessel walls, 13  that CRP avidly binds to human neutrophils, 14  and that CRP can induce complement activation.	bind
20200	2	6457	5	NULL	NULL	0	NULL	CRP	NULL		bind	NULL	avidly			neutrophils	NULL	human			NULL		0	NULL	NULL	NULL	gw60_circulation_97_5_425_s_78	9490235	12  Experimental work also suggests that CRP can be found within endothelial vessel walls, 13  that CRP avidly binds to human neutrophils, 14  and that CRP can induce complement activation.	bind
20201	3	6457	5	NULL	NULL	0	NULL	CRP	NULL		induces	NULL				complement	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_circulation_97_5_425_s_78	9490235	12  Experimental work also suggests that CRP can be found within endothelial vessel walls, 13  that CRP avidly binds to human neutrophils, 14  and that CRP can induce complement activation.	bind
23624	1	6457	7	NULL	NULL	NULL	NULL	CRP	GP		is found within					endothelial vessel walls	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_5_425_s_78	9490235	12  Experimental work also suggests that CRP can be found within endothelial vessel walls, 13  that CRP avidly binds to human neutrophils, 14  and that CRP can induce complement activation.	bind
23625	2	6457	7	NULL	NULL	NULL	NULL	CRP	GP		binds		avidly			neutrophils	Cell	human			NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_5_425_s_78	9490235	12  Experimental work also suggests that CRP can be found within endothelial vessel walls, 13  that CRP avidly binds to human neutrophils, 14  and that CRP can induce complement activation.	bind
23626	3	6457	7	NULL	NULL	NULL	NULL	CRP	GP		induce					complement	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_5_425_s_78	9490235	12  Experimental work also suggests that CRP can be found within endothelial vessel walls, 13  that CRP avidly binds to human neutrophils, 14  and that CRP can induce complement activation.	bind
20202	1	6458	5	NULL	NULL	0	NULL	apoB	NULL		bind	NULL				LDLR	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_6_794_s_195	8640407	12  However, according to the direct binding assays in this study, we found no evidence for altered binding of apoB or apoE to the LDLR of pattern B subjects, consistent with recent evidence (J.K. Naggert et al, unpublished data, 1995) of the absence of functional mutations in the structural position of the LDLR gene in pattern B subjects.	bind
20203	2	6458	5	NULL	NULL	0	NULL	apoE	NULL		bind	NULL				LDLR	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_6_794_s_195	8640407	12  However, according to the direct binding assays in this study, we found no evidence for altered binding of apoB or apoE to the LDLR of pattern B subjects, consistent with recent evidence (J.K. Naggert et al, unpublished data, 1995) of the absence of functional mutations in the structural position of the LDLR gene in pattern B subjects.	bind
20204	3	6458	5	NULL	NULL	0	NULL	functional mutations	NULL		is absent in	NULL				LDLR gene	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_6_794_s_195	8640407	12  However, according to the direct binding assays in this study, we found no evidence for altered binding of apoB or apoE to the LDLR of pattern B subjects, consistent with recent evidence (J.K. Naggert et al, unpublished data, 1995) of the absence of functional mutations in the structural position of the LDLR gene in pattern B subjects.	bind
23633	1	6458	7	NULL	NULL	NULL	NULL	apoB	GP		bind					LDLR	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_6_794_s_195	8640407	12  However, according to the direct binding assays in this study, we found no evidence for altered binding of apoB or apoE to the LDLR of pattern B subjects, consistent with recent evidence (J.K. Naggert et al, unpublished data, 1995) of the absence of functional mutations in the structural position of the LDLR gene in pattern B subjects.	bind
23634	2	6458	7	NULL	NULL	NULL	NULL	apoE	GP		bind					LDLR	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_6_794_s_195	8640407	12  However, according to the direct binding assays in this study, we found no evidence for altered binding of apoB or apoE to the LDLR of pattern B subjects, consistent with recent evidence (J.K. Naggert et al, unpublished data, 1995) of the absence of functional mutations in the structural position of the LDLR gene in pattern B subjects.	bind
30857	3	6458	7	NULL	NULL	NULL	NULL	functional mutation	Process		is absent in					LDLR gene	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_6_794_s_195	8640407	12  However, according to the direct binding assays in this study, we found no evidence for altered binding of apoB or apoE to the LDLR of pattern B subjects, consistent with recent evidence (J.K. Naggert et al, unpublished data, 1995) of the absence of functional mutations in the structural position of the LDLR gene in pattern B subjects.	bind
20205	1	6459	5	NULL	NULL	0	NULL	CRP	NULL		bind	NULL	low affinity			FCgammaRI	NULL				NULL	on leukocytes	NULL	NULL	NULL	NULL	gw60_circulation_102_18_2165_s_83	11056086	12  In addition, recent studies 13  have shown that CRP can bind to receptor FCgammaRI (with low affinity) and FCgammaRII (with high affinity) on leukocytes.	bind
20206	2	6459	5	NULL	NULL	0	NULL	CRP	NULL		bind	NULL	high affinity			FCgammaRII	NULL				NULL	on leukocytes	NULL	NULL	NULL	NULL	gw60_circulation_102_18_2165_s_83	11056086	12  In addition, recent studies 13  have shown that CRP can bind to receptor FCgammaRI (with low affinity) and FCgammaRII (with high affinity) on leukocytes.	bind
30033	3	6459	5	NULL	NULL	0	NULL	FCgammaRI	NULL		is a type of	NULL				receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_102_18_2165_s_83	11056086	12  In addition, recent studies 13  have shown that CRP can bind to receptor FCgammaRI (with low affinity) and FCgammaRII (with high affinity) on leukocytes.	bind
30034	4	6459	5	NULL	NULL	0	NULL	FCgammaRII	NULL		is a type of	NULL				receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_102_18_2165_s_83	11056086	12  In addition, recent studies 13  have shown that CRP can bind to receptor FCgammaRI (with low affinity) and FCgammaRII (with high affinity) on leukocytes.	bind
23638	1	6459	7	NULL	NULL	NULL	NULL	CRP	GP		bind		low affinity			FCgammaRI	GP				NULL	leukocytes	NULL	NULL	NULL	NULL	gw60_circulation_102_18_2165_s_83	11056086	12  In addition, recent studies 13  have shown that CRP can bind to receptor FCgammaRI (with low affinity) and FCgammaRII (with high affinity) on leukocytes.	bind
23641	2	6459	7	NULL	NULL	NULL	NULL	CRP	GP		bind		high affinity			 FCgammaRII 	GP				NULL	leukocytes	NULL	NULL	NULL	NULL	gw60_circulation_102_18_2165_s_83	11056086	12  In addition, recent studies 13  have shown that CRP can bind to receptor FCgammaRI (with low affinity) and FCgammaRII (with high affinity) on leukocytes.	bind
30867	3	6459	7	NULL	NULL	NULL	NULL	FCgammaRI	GP		is a type of					receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_18_2165_s_83	11056086	12  In addition, recent studies 13  have shown that CRP can bind to receptor FCgammaRI (with low affinity) and FCgammaRII (with high affinity) on leukocytes.	bind
30869	4	6459	7	NULL	NULL	NULL	NULL	FCgammaRII	GP		is a type of					receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_18_2165_s_83	11056086	12  In addition, recent studies 13  have shown that CRP can bind to receptor FCgammaRI (with low affinity) and FCgammaRII (with high affinity) on leukocytes.	bind
20207	1	6460	5	10	NULL	0	NULL	Egr-1			bind					PDGF-A - chain				promoter	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_6_678_s_243	10189355	12  In these studies, the binding of Egr-1 to the PDGF-A - chain promoter was induced by shear stress, which displaced SP-1 from their overlapping recognition elements.	bind
20208	2	6460	5	NULL	NULL	0	NULL	shear stress	NULL		induces	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_6_678_s_243	10189355	12  In these studies, the binding of Egr-1 to the PDGF-A - chain promoter was induced by shear stress, which displaced SP-1 from their overlapping recognition elements.	bind
20209	3	6460	5	10	NULL	0	NULL	SP-1	NULL		is displaced from	NULL					NULL			overlapping recognition elements	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_6_678_s_243	10189355	12  In these studies, the binding of Egr-1 to the PDGF-A - chain promoter was induced by shear stress, which displaced SP-1 from their overlapping recognition elements.	bind
20210	4	6460	5	NULL	NULL	0	NULL	statement 1	NULL		results in	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_6_678_s_243	10189355	12  In these studies, the binding of Egr-1 to the PDGF-A - chain promoter was induced by shear stress, which displaced SP-1 from their overlapping recognition elements.	bind
23644	1	6460	7	NULL	NULL	NULL	NULL	Egr-1 	GP		bind					PDGF-A - chain	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_6_678_s_243	10189355	12  In these studies, the binding of Egr-1 to the PDGF-A - chain promoter was induced by shear stress, which displaced SP-1 from their overlapping recognition elements.	bind
23646	2	6460	7	NULL	NULL	NULL	NULL	shear stress	Process		induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_6_678_s_243	10189355	12  In these studies, the binding of Egr-1 to the PDGF-A - chain promoter was induced by shear stress, which displaced SP-1 from their overlapping recognition elements.	bind
23651	3	6460	7	NULL	NULL	NULL	NULL	SP-1	GP		is displaced from									overlapping recognition elements	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_6_678_s_243	10189355	12  In these studies, the binding of Egr-1 to the PDGF-A - chain promoter was induced by shear stress, which displaced SP-1 from their overlapping recognition elements.	bind
30872	4	6460	7	NULL	NULL	NULL	NULL	statement 1	Process		results in					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_6_678_s_243	10189355	12  In these studies, the binding of Egr-1 to the PDGF-A - chain promoter was induced by shear stress, which displaced SP-1 from their overlapping recognition elements.	bind
20211	1	6461	5	NULL	NULL	0	NULL	IP-10	NULL		is a ligand for	NULL	major			CXCR3	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_3_1053_s_222	11238053	12  IP-10 is a major ligand for CXCR3, suggesting its involvement in type 1 cell recruitment, whereas eotaxin and MDC bind preferentially CCR3 and CCR4, respectively, suggesting an activity on type 2 cells.	bind
20212	2	6461	5	NULL	NULL	0	NULL	 IP-10	NULL		is involved in	NULL				type 1 cell 	NULL	recruitment of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_3_1053_s_222	11238053	12  IP-10 is a major ligand for CXCR3, suggesting its involvement in type 1 cell recruitment, whereas eotaxin and MDC bind preferentially CCR3 and CCR4, respectively, suggesting an activity on type 2 cells.	bind
20213	3	6461	5	NULL	NULL	0	NULL	statement 1	NULL		suggests	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_3_1053_s_222	11238053	12  IP-10 is a major ligand for CXCR3, suggesting its involvement in type 1 cell recruitment, whereas eotaxin and MDC bind preferentially CCR3 and CCR4, respectively, suggesting an activity on type 2 cells.	bind
20215	4	6461	5	NULL	NULL	0	NULL	eotaxin	NULL		bind	NULL	preferentially			CCR3	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_3_1053_s_222	11238053	12  IP-10 is a major ligand for CXCR3, suggesting its involvement in type 1 cell recruitment, whereas eotaxin and MDC bind preferentially CCR3 and CCR4, respectively, suggesting an activity on type 2 cells.	bind
20216	5	6461	5	NULL	NULL	0	NULL	MDC	NULL		bind	NULL	preferentially			CCR4	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_3_1053_s_222	11238053	12  IP-10 is a major ligand for CXCR3, suggesting its involvement in type 1 cell recruitment, whereas eotaxin and MDC bind preferentially CCR3 and CCR4, respectively, suggesting an activity on type 2 cells.	bind
20217	6	6461	5	NULL	NULL	0	NULL	statement 4	NULL		suggests	NULL				type 2 cells	NULL	activity on			NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_3_1053_s_222	11238053	12  IP-10 is a major ligand for CXCR3, suggesting its involvement in type 1 cell recruitment, whereas eotaxin and MDC bind preferentially CCR3 and CCR4, respectively, suggesting an activity on type 2 cells.	bind
20218	7	6461	5	NULL	NULL	0	NULL	statement 5	NULL		suggests	NULL				type 2 cells	NULL	activity on			NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_3_1053_s_222	11238053	12  IP-10 is a major ligand for CXCR3, suggesting its involvement in type 1 cell recruitment, whereas eotaxin and MDC bind preferentially CCR3 and CCR4, respectively, suggesting an activity on type 2 cells.	bind
23665	1	6461	7	NULL	NULL	NULL	NULL	IP-10	GP		is a ligand for					CXCR3	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_3_1053_s_222	11238053	12  IP-10 is a major ligand for CXCR3, suggesting its involvement in type 1 cell recruitment, whereas eotaxin and MDC bind preferentially CCR3 and CCR4, respectively, suggesting an activity on type 2 cells.	bind
23669	2	6461	7	NULL	NULL	NULL	NULL	statement 1	Process		involve in					type 1 cell 	Cell	recruitment of 			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_3_1053_s_222	11238053	12  IP-10 is a major ligand for CXCR3, suggesting its involvement in type 1 cell recruitment, whereas eotaxin and MDC bind preferentially CCR3 and CCR4, respectively, suggesting an activity on type 2 cells.	bind
23670	3	6461	7	NULL	NULL	NULL	NULL	eotaxin	GP		bind		preferentially			CCR3	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_3_1053_s_222	11238053	12  IP-10 is a major ligand for CXCR3, suggesting its involvement in type 1 cell recruitment, whereas eotaxin and MDC bind preferentially CCR3 and CCR4, respectively, suggesting an activity on type 2 cells.	bind
23671	4	6461	7	NULL	NULL	NULL	NULL	MDC	GP		bind		preferentially			CCR4	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_3_1053_s_222	11238053	12  IP-10 is a major ligand for CXCR3, suggesting its involvement in type 1 cell recruitment, whereas eotaxin and MDC bind preferentially CCR3 and CCR4, respectively, suggesting an activity on type 2 cells.	bind
23676	5	6461	7	NULL	NULL	NULL	NULL	statement 3	Process		suggests					type 2 cells	Cell	activity on			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_3_1053_s_222	11238053	12  IP-10 is a major ligand for CXCR3, suggesting its involvement in type 1 cell recruitment, whereas eotaxin and MDC bind preferentially CCR3 and CCR4, respectively, suggesting an activity on type 2 cells.	bind
23679	6	6461	7	NULL	NULL	NULL	NULL	statement 4	Process		suggests					type 2 cells	Cell	activity on			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_3_1053_s_222	11238053	12  IP-10 is a major ligand for CXCR3, suggesting its involvement in type 1 cell recruitment, whereas eotaxin and MDC bind preferentially CCR3 and CCR4, respectively, suggesting an activity on type 2 cells.	bind
30873	7	6461	7	NULL	NULL	NULL	NULL	statement 1	Process		suggests					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_3_1053_s_222	11238053	12  IP-10 is a major ligand for CXCR3, suggesting its involvement in type 1 cell recruitment, whereas eotaxin and MDC bind preferentially CCR3 and CCR4, respectively, suggesting an activity on type 2 cells.	bind
20219	1	6462	5	NULL	NULL	0	NULL	PAI-1	NULL		bind	NULL				vitronectin	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_11_2037_s_28	7583587	12  PAI-1 bound to vitronectin in the matrix is known to be a spreading factor for several cell types.	bind
30035	2	6462	5	NULL	NULL	0	NULL	statement 1	NULL		is a type of	NULL				spreading factor	NULL				NULL	several cell types	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_11_2037_s_28	7583587	12  PAI-1 bound to vitronectin in the matrix is known to be a spreading factor for several cell types.	bind
23683	1	6462	7	NULL	NULL	NULL	NULL	PAI-1	GP		bind					vitronectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_11_2037_s_28	7583587	12  PAI-1 bound to vitronectin in the matrix is known to be a spreading factor for several cell types.	bind
23686	2	6462	7	NULL	NULL	NULL	NULL	statement 1	Process		is a type of					spreading factor	Process				NULL	several cell types	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_11_2037_s_28	7583587	12  PAI-1 bound to vitronectin in the matrix is known to be a spreading factor for several cell types.	bind
20220	1	6463	5	NULL	NULL	0	NULL	SRF	NULL		bind	NULL					NULL			CArG A	NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2049_s_158	10479645	12  Taken together, these data indicate that TGF-beta - induced increases in SRF binding to CArG A and B were much greater in SMCs than non-SMCs and that SRF binding activities are regulated in a cell-specific manner.	bind
20221	2	6463	5	NULL	NULL	0	NULL	SRF	NULL		bind	NULL					NULL			CArG B	NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2049_s_158	10479645	12  Taken together, these data indicate that TGF-beta - induced increases in SRF binding to CArG A and B were much greater in SMCs than non-SMCs and that SRF binding activities are regulated in a cell-specific manner.	bind
20222	3	6463	5	NULL	NULL	0	NULL	TGF-beta	NULL	induced	increases	NULL				statement 1	NULL				NULL	in SMCs	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2049_s_158	10479645	12  Taken together, these data indicate that TGF-beta - induced increases in SRF binding to CArG A and B were much greater in SMCs than non-SMCs and that SRF binding activities are regulated in a cell-specific manner.	bind
20223	4	6463	5	NULL	NULL	0	NULL	TGF-beta	NULL	induced	increases	NULL				statement 2	NULL				NULL	in SMCs	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2049_s_158	10479645	12  Taken together, these data indicate that TGF-beta - induced increases in SRF binding to CArG A and B were much greater in SMCs than non-SMCs and that SRF binding activities are regulated in a cell-specific manner.	bind
20224	5	6463	5	NULL	NULL	0	NULL	TGF-beta	NULL	induced	increases	NULL				statement 1	NULL				NULL	in non-SMCs	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2049_s_158	10479645	12  Taken together, these data indicate that TGF-beta - induced increases in SRF binding to CArG A and B were much greater in SMCs than non-SMCs and that SRF binding activities are regulated in a cell-specific manner.	bind
20225	6	6463	5	NULL	NULL	0	NULL	TGF-beta	NULL	induced	increases	NULL				statement 2	NULL				NULL	in non-SMCs	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2049_s_158	10479645	12  Taken together, these data indicate that TGF-beta - induced increases in SRF binding to CArG A and B were much greater in SMCs than non-SMCs and that SRF binding activities are regulated in a cell-specific manner.	bind
20226	7	6463	5	NULL	NULL	0	NULL	statement 3	NULL		greater than	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2049_s_158	10479645	12  Taken together, these data indicate that TGF-beta - induced increases in SRF binding to CArG A and B were much greater in SMCs than non-SMCs and that SRF binding activities are regulated in a cell-specific manner.	bind
20227	8	6463	5	NULL	NULL	0	NULL	statement 4	NULL		greater than	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2049_s_158	10479645	12  Taken together, these data indicate that TGF-beta - induced increases in SRF binding to CArG A and B were much greater in SMCs than non-SMCs and that SRF binding activities are regulated in a cell-specific manner.	bind
20228	9	6463	5	NULL	NULL	0	NULL	SRF	NULL	binding activities	is regulated in	NULL				cell-specific manner	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2049_s_158	10479645	12  Taken together, these data indicate that TGF-beta - induced increases in SRF binding to CArG A and B were much greater in SMCs than non-SMCs and that SRF binding activities are regulated in a cell-specific manner.	bind
23688	1	6463	7	NULL	NULL	NULL	NULL	SRF	GP		bind									CArG A	NULL	SMCs	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2049_s_158	10479645	12  Taken together, these data indicate that TGF-beta - induced increases in SRF binding to CArG A and B were much greater in SMCs than non-SMCs and that SRF binding activities are regulated in a cell-specific manner.	bind
23689	2	6463	7	NULL	NULL	NULL	NULL	SRF	GP		bind									CArG B	NULL	SMCs	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2049_s_158	10479645	12  Taken together, these data indicate that TGF-beta - induced increases in SRF binding to CArG A and B were much greater in SMCs than non-SMCs and that SRF binding activities are regulated in a cell-specific manner.	bind
23690	3	6463	7	NULL	NULL	NULL	NULL	SRF	GP		bind									CArG A	NULL	non-SMCs	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2049_s_158	10479645	12  Taken together, these data indicate that TGF-beta - induced increases in SRF binding to CArG A and B were much greater in SMCs than non-SMCs and that SRF binding activities are regulated in a cell-specific manner.	bind
23691	4	6463	7	NULL	NULL	NULL	NULL	SRF	GP		bind									CArG B	NULL	non-SMCs	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2049_s_158	10479645	12  Taken together, these data indicate that TGF-beta - induced increases in SRF binding to CArG A and B were much greater in SMCs than non-SMCs and that SRF binding activities are regulated in a cell-specific manner.	bind
23692	5	6463	7	NULL	NULL	NULL	NULL	TGF-beta	GP	induced	increase					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2049_s_158	10479645	12  Taken together, these data indicate that TGF-beta - induced increases in SRF binding to CArG A and B were much greater in SMCs than non-SMCs and that SRF binding activities are regulated in a cell-specific manner.	bind
23693	6	6463	7	NULL	NULL	NULL	NULL	TGF-beta	GP	induced	increase					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2049_s_158	10479645	12  Taken together, these data indicate that TGF-beta - induced increases in SRF binding to CArG A and B were much greater in SMCs than non-SMCs and that SRF binding activities are regulated in a cell-specific manner.	bind
23694	7	6463	7	NULL	NULL	NULL	NULL	TGF-beta	GP	induced	increase					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2049_s_158	10479645	12  Taken together, these data indicate that TGF-beta - induced increases in SRF binding to CArG A and B were much greater in SMCs than non-SMCs and that SRF binding activities are regulated in a cell-specific manner.	bind
23695	8	6463	7	NULL	NULL	NULL	NULL	TGF-beta	GP	induced	increase					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2049_s_158	10479645	12  Taken together, these data indicate that TGF-beta - induced increases in SRF binding to CArG A and B were much greater in SMCs than non-SMCs and that SRF binding activities are regulated in a cell-specific manner.	bind
23696	9	6463	7	NULL	NULL	NULL	NULL	statement 5	Process		is greater than					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2049_s_158	10479645	12  Taken together, these data indicate that TGF-beta - induced increases in SRF binding to CArG A and B were much greater in SMCs than non-SMCs and that SRF binding activities are regulated in a cell-specific manner.	bind
23697	10	6463	7	NULL	NULL	NULL	NULL	statement 6	Process		is greater than					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2049_s_158	10479645	12  Taken together, these data indicate that TGF-beta - induced increases in SRF binding to CArG A and B were much greater in SMCs than non-SMCs and that SRF binding activities are regulated in a cell-specific manner.	bind
20229	1	6464	5	NULL	NULL	0	NULL	fibrinogen	NULL		bind	NULL				GP IIb/IIIa receptors	NULL				NULL	on activated platelets	0	NULL	NULL	NULL	gw60_circulation_98_8_813_s_172	9727553	12  The binding of fibrinogen to GP IIb/IIIa receptors on activated platelets represents the final common pathway for platelet aggregation.	bind
20230	2	6464	5	NULL	NULL	0	NULL	statement 1	NULL		represents	NULL				platelet aggregation	NULL	final common pathway for			NULL		0	NULL	NULL	NULL	gw60_circulation_98_8_813_s_172	9727553	12  The binding of fibrinogen to GP IIb/IIIa receptors on activated platelets represents the final common pathway for platelet aggregation.	bind
23698	1	6464	7	NULL	NULL	NULL	NULL	fibrinogen	GP		bind					GP IIb/IIIa receptors 	GP				NULL	activated platelets	NULL	NULL	NULL	NULL	gw60_circulation_98_8_813_s_172	9727553	12  The binding of fibrinogen to GP IIb/IIIa receptors on activated platelets represents the final common pathway for platelet aggregation.	bind
23699	2	6464	7	NULL	NULL	NULL	NULL	statement 1	Process		represent					platelet aggregation	Process	final common pathway for			NULL		NULL	NULL	NULL	NULL	gw60_circulation_98_8_813_s_172	9727553	12  The binding of fibrinogen to GP IIb/IIIa receptors on activated platelets represents the final common pathway for platelet aggregation.	bind
20231	1	6465	5	10	NULL	0	NULL	CN-Cbl	NULL		is not 	NULL				Cbl	NULL	biologically active form of 			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2074_s_39	9351374	12 13  CN-Cbl is not the biologically active form of Cbl; CN-Cbl must be converted to aqCbl to become a precursor of the Cbl II that is bound by apo-methionine synthase (Fig 1  ).	bind
20232	2	6465	5	10	NULL	0	NULL	CN-Cbl	NULL		is converted to	NULL				aqCbl	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2074_s_39	9351374	12 13  CN-Cbl is not the biologically active form of Cbl; CN-Cbl must be converted to aqCbl to become a precursor of the Cbl II that is bound by apo-methionine synthase (Fig 1  ).	bind
20233	4	6465	5	10	NULL	0	NULL	aqCbl	NULL		becomes	NULL				statement 3	NULL	precursor of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2074_s_39	9351374	12 13  CN-Cbl is not the biologically active form of Cbl; CN-Cbl must be converted to aqCbl to become a precursor of the Cbl II that is bound by apo-methionine synthase (Fig 1  ).	bind
20234	3	6465	5	NULL	NULL	0	NULL	Cbl II	NULL		bind	NULL				apo-methionine synthase	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2074_s_39	9351374	12 13  CN-Cbl is not the biologically active form of Cbl; CN-Cbl must be converted to aqCbl to become a precursor of the Cbl II that is bound by apo-methionine synthase (Fig 1  ).	bind
23700	1	6465	7	NULL	NULL	NULL	NULL	CN-Cbl	Chemical		is not					Cbl	Chemical	biologically active form of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2074_s_39	9351374	12 13  CN-Cbl is not the biologically active form of Cbl; CN-Cbl must be converted to aqCbl to become a precursor of the Cbl II that is bound by apo-methionine synthase (Fig 1  ).	bind
23701	2	6465	7	NULL	NULL	NULL	NULL	CN-Cbl	Chemical		is converted to					aqCbl	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2074_s_39	9351374	12 13  CN-Cbl is not the biologically active form of Cbl; CN-Cbl must be converted to aqCbl to become a precursor of the Cbl II that is bound by apo-methionine synthase (Fig 1  ).	bind
23702	3	6465	7	NULL	NULL	NULL	NULL	statement 2	Process		is a precursor of					Cbl II	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2074_s_39	9351374	12 13  CN-Cbl is not the biologically active form of Cbl; CN-Cbl must be converted to aqCbl to become a precursor of the Cbl II that is bound by apo-methionine synthase (Fig 1  ).	bind
23703	4	6465	7	NULL	NULL	NULL	NULL	apo-methionine synthase	GP		bind					Cbl II	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2074_s_39	9351374	12 13  CN-Cbl is not the biologically active form of Cbl; CN-Cbl must be converted to aqCbl to become a precursor of the Cbl II that is bound by apo-methionine synthase (Fig 1  ).	bind
20235	1	6466	5	NULL	NULL	0	NULL	CETP	NULL		bind	NULL				HDL cholesteryl ester	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_102_18_2197_s_117	11056092	12 13 14  An amino acid substitution such as the present (resulting in loss of positive charge at this position) could therefore influence the binding of CETP to HDL cholesteryl ester and thereby indirectly affect the efficiency of the protein transferring cholesteryl ester out of HDL particles.	bind
20236	2	6466	5	10	NULL	0	NULL	amino acid		substitution	influence					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_18_2197_s_117	11056092	12 13 14  An amino acid substitution such as the present (resulting in loss of positive charge at this position) could therefore influence the binding of CETP to HDL cholesteryl ester and thereby indirectly affect the efficiency of the protein transferring cholesteryl ester out of HDL particles.	bind
20237	4	6466	5	NULL	NULL	0	NULL	statement 2	NULL		affect	NULL	indirectly			statement 3	NULL	efficiency of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_18_2197_s_117	11056092	12 13 14  An amino acid substitution such as the present (resulting in loss of positive charge at this position) could therefore influence the binding of CETP to HDL cholesteryl ester and thereby indirectly affect the efficiency of the protein transferring cholesteryl ester out of HDL particles.	bind
46190	3	6466	5	NULL	NULL	0	NULL	cholesteryl ester	NULL		is transferred out of	NULL				HDL particles	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_102_18_2197_s_117	11056092	12 13 14  An amino acid substitution such as the present (resulting in loss of positive charge at this position) could therefore influence the binding of CETP to HDL cholesteryl ester and thereby indirectly affect the efficiency of the protein transferring cholesteryl ester out of HDL particles.	bind
23704	1	6466	7	NULL	NULL	NULL	NULL	CETP 	GP		bind					HDL cholesteryl ester	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_18_2197_s_117	11056092	12 13 14  An amino acid substitution such as the present (resulting in loss of positive charge at this position) could therefore influence the binding of CETP to HDL cholesteryl ester and thereby indirectly affect the efficiency of the protein transferring cholesteryl ester out of HDL particles.	bind
23705	2	6466	7	NULL	NULL	NULL	NULL	aminoacid	AminoAcid	substitution	influence					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_18_2197_s_117	11056092	12 13 14  An amino acid substitution such as the present (resulting in loss of positive charge at this position) could therefore influence the binding of CETP to HDL cholesteryl ester and thereby indirectly affect the efficiency of the protein transferring cholesteryl ester out of HDL particles.	bind
23706	3	6466	7	NULL	NULL	NULL	NULL	cholesteryl ester	Chemical		is transferred out of					HDL particles	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_18_2197_s_117	11056092	12 13 14  An amino acid substitution such as the present (resulting in loss of positive charge at this position) could therefore influence the binding of CETP to HDL cholesteryl ester and thereby indirectly affect the efficiency of the protein transferring cholesteryl ester out of HDL particles.	bind
45753	4	6466	7	NULL	NULL	NULL	NULL	statement 2	Process		affect 		indirectly			statement 3	Process	efficiency of protein of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_18_2197_s_117	11056092	12 13 14  An amino acid substitution such as the present (resulting in loss of positive charge at this position) could therefore influence the binding of CETP to HDL cholesteryl ester and thereby indirectly affect the efficiency of the protein transferring cholesteryl ester out of HDL particles.	bind
20238	1	6467	5	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				Ral	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_899_s_108	11397694	12 15  Recently, a binding site for calmodulin on Ral has been detected, and calmodulin has been shown to enhance the binding of GTP to Ral. 23  24  We investigated whether thrombin-induced activation of Ral is affected by antagonists of calmodulin.	bind
20239	2	6467	5	NULL	NULL	0	NULL	calmodulin	NULL		enhances	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_899_s_108	11397694	12 15  Recently, a binding site for calmodulin on Ral has been detected, and calmodulin has been shown to enhance the binding of GTP to Ral. 23  24  We investigated whether thrombin-induced activation of Ral is affected by antagonists of calmodulin.	bind
45623	3	6467	5	10	NULL	0	NULL	thrombin	NULL		induce	NULL				Ral	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_899_s_108	11397694	12 15  Recently, a binding site for calmodulin on Ral has been detected, and calmodulin has been shown to enhance the binding of GTP to Ral. 23  24  We investigated whether thrombin-induced activation of Ral is affected by antagonists of calmodulin.	bind
23839	1	6467	7	NULL	NULL	NULL	NULL	GTP	Chemical		bind					Ral	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_899_s_108	11397694	12 15  Recently, a binding site for calmodulin on Ral has been detected, and calmodulin has been shown to enhance the binding of GTP to Ral. 23  24  We investigated whether thrombin-induced activation of Ral is affected by antagonists of calmodulin.	bind
23840	2	6467	7	NULL	NULL	NULL	NULL	calmodulin	GP		enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_899_s_108	11397694	12 15  Recently, a binding site for calmodulin on Ral has been detected, and calmodulin has been shown to enhance the binding of GTP to Ral. 23  24  We investigated whether thrombin-induced activation of Ral is affected by antagonists of calmodulin.	bind
23841	3	6467	7	NULL	NULL	NULL	NULL	thrombin	GP		induce					Ral	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_899_s_108	11397694	12 15  Recently, a binding site for calmodulin on Ral has been detected, and calmodulin has been shown to enhance the binding of GTP to Ral. 23  24  We investigated whether thrombin-induced activation of Ral is affected by antagonists of calmodulin.	bind
23842	4	6467	7	NULL	NULL	NULL	NULL	Ral	GP		contain								calmodulin binding site		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_899_s_108	11397694	12 15  Recently, a binding site for calmodulin on Ral has been detected, and calmodulin has been shown to enhance the binding of GTP to Ral. 23  24  We investigated whether thrombin-induced activation of Ral is affected by antagonists of calmodulin.	bind
20240	1	6469	5	NULL	NULL	0	NULL	glucocorticoids	NULL		up-regulates	NULL				HDL-specific binding	NULL				NULL	rat hepatocytes	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_6_1143_s_213	9194766	12 57  Moreover, despite earlier published data showed that glucocorticoids can upregulate HDL-specific binding in rat hepatocytes, 58  in our experiments Dex had no effect on specific binding of HDL3 to cultured SMC (Table 6  ).	bind
20241	2	6469	5	NULL	NULL	0	NULL	HDL3	NULL		bind	NULL	specifically			SMC	NULL	cultured			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_6_1143_s_213	9194766	12 57  Moreover, despite earlier published data showed that glucocorticoids can upregulate HDL-specific binding in rat hepatocytes, 58  in our experiments Dex had no effect on specific binding of HDL3 to cultured SMC (Table 6  ).	bind
20242	3	6469	5	NULL	NULL	0	NULL	Dex	NULL		does not effect	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_6_1143_s_213	9194766	12 57  Moreover, despite earlier published data showed that glucocorticoids can upregulate HDL-specific binding in rat hepatocytes, 58  in our experiments Dex had no effect on specific binding of HDL3 to cultured SMC (Table 6  ).	bind
23844	1	6469	7	NULL	NULL	NULL	NULL	 glucocorticoids	Chemical		upregulate					HDL-specific binding	Process				NULL	rat hepatocytes	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_6_1143_s_213	9194766	12 57  Moreover, despite earlier published data showed that glucocorticoids can upregulate HDL-specific binding in rat hepatocytes, 58  in our experiments Dex had no effect on specific binding of HDL3 to cultured SMC (Table 6  ).	bind
23845	2	6469	7	NULL	NULL	NULL	NULL	HDL3	GP		bind					SMC	Cell	cultured 			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_6_1143_s_213	9194766	12 57  Moreover, despite earlier published data showed that glucocorticoids can upregulate HDL-specific binding in rat hepatocytes, 58  in our experiments Dex had no effect on specific binding of HDL3 to cultured SMC (Table 6  ).	bind
23846	3	6469	7	NULL	NULL	NULL	NULL	Dex	Chemical		does not effect					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_6_1143_s_213	9194766	12 57  Moreover, despite earlier published data showed that glucocorticoids can upregulate HDL-specific binding in rat hepatocytes, 58  in our experiments Dex had no effect on specific binding of HDL3 to cultured SMC (Table 6  ).	bind
20243	1	6471	5	NULL	NULL	0	NULL	E7	NULL		bind	NULL				Rb	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_162_6_1789_s_20	12759237	12 E7 binds to the retinoblastoma protein Rb, and disrupts the complex between Rb and the E2F transcription factor family, which controls the expression of genes involved in cell-cycle progression.	bind
20244	2	6471	5	NULL	NULL	0	NULL	Rb	NULL		is	NULL				retinoblastoma protein	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_162_6_1789_s_20	12759237	12 E7 binds to the retinoblastoma protein Rb, and disrupts the complex between Rb and the E2F transcription factor family, which controls the expression of genes involved in cell-cycle progression.	bind
20245	3	6471	5	NULL	NULL	0	NULL	Rb	NULL		complexes with	NULL				E2F transcription factor family	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_162_6_1789_s_20	12759237	12 E7 binds to the retinoblastoma protein Rb, and disrupts the complex between Rb and the E2F transcription factor family, which controls the expression of genes involved in cell-cycle progression.	bind
20246	4	6471	5	NULL	NULL	0	NULL	statement 1	NULL		disrupts	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_162_6_1789_s_20	12759237	12 E7 binds to the retinoblastoma protein Rb, and disrupts the complex between Rb and the E2F transcription factor family, which controls the expression of genes involved in cell-cycle progression.	bind
20247	5	6471	5	NULL	NULL	0	NULL	statement 4	NULL		controls	NULL				genes involved in cell-cycle progression	NULL	expression of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_162_6_1789_s_20	12759237	12 E7 binds to the retinoblastoma protein Rb, and disrupts the complex between Rb and the E2F transcription factor family, which controls the expression of genes involved in cell-cycle progression.	bind
23847	1	6471	7	NULL	NULL	NULL	NULL	E7	GP		binds to					Rb	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_162_6_1789_s_20	12759237	12 E7 binds to the retinoblastoma protein Rb, and disrupts the complex between Rb and the E2F transcription factor family, which controls the expression of genes involved in cell-cycle progression.	bind
23848	2	6471	7	NULL	NULL	NULL	NULL	Rb	GP		complex with					transcription factor family E2F	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_162_6_1789_s_20	12759237	12 E7 binds to the retinoblastoma protein Rb, and disrupts the complex between Rb and the E2F transcription factor family, which controls the expression of genes involved in cell-cycle progression.	bind
23849	3	6471	7	NULL	NULL	NULL	NULL	statement 1	Process		disrupts					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_162_6_1789_s_20	12759237	12 E7 binds to the retinoblastoma protein Rb, and disrupts the complex between Rb and the E2F transcription factor family, which controls the expression of genes involved in cell-cycle progression.	bind
23850	4	6471	7	NULL	NULL	NULL	NULL	E2F	GP		controls					genes involved in cell-cycle progression	GP	expression of 			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_162_6_1789_s_20	12759237	12 E7 binds to the retinoblastoma protein Rb, and disrupts the complex between Rb and the E2F transcription factor family, which controls the expression of genes involved in cell-cycle progression.	bind
30878	5	6471	7	NULL	NULL	NULL	NULL	Rb	GP		is					retinoblastoma protein 	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_162_6_1789_s_20	12759237	12 E7 binds to the retinoblastoma protein Rb, and disrupts the complex between Rb and the E2F transcription factor family, which controls the expression of genes involved in cell-cycle progression.	bind
20248	1	6472	5	NULL	NULL	0	NULL	Notch	NULL		mediate	NULL				SMA	NULL	upregulation of 			NULL		0	NULL	NULL	NULL	gw70_circulationres_98_12_1468_s_25	16741155	12 Here we demonstrate that Notch-mediated upregulation of SMA is directly dependent on the activation and binding of CSL to the SMA promoter.	bind
20249	2	6472	5	NULL	NULL	0	NULL	CSL	NULL		bind	NULL				SMA	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_circulationres_98_12_1468_s_25	16741155	12 Here we demonstrate that Notch-mediated upregulation of SMA is directly dependent on the activation and binding of CSL to the SMA promoter.	bind
20250	3	6472	5	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL	directly			CSL	NULL	activation of			NULL		0	NULL	NULL	NULL	gw70_circulationres_98_12_1468_s_25	16741155	12 Here we demonstrate that Notch-mediated upregulation of SMA is directly dependent on the activation and binding of CSL to the SMA promoter.	bind
20251	4	6472	5	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL	directly			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_12_1468_s_25	16741155	12 Here we demonstrate that Notch-mediated upregulation of SMA is directly dependent on the activation and binding of CSL to the SMA promoter.	bind
23851	1	6472	7	NULL	NULL	NULL	NULL	CSL 	GP		bind					SMA	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_12_1468_s_25	16741155	12 Here we demonstrate that Notch-mediated upregulation of SMA is directly dependent on the activation and binding of CSL to the SMA promoter.	bind
23852	2	6472	7	NULL	NULL	NULL	NULL	Notch	GP		mediates					SMA	GP	upregulation of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_12_1468_s_25	16741155	12 Here we demonstrate that Notch-mediated upregulation of SMA is directly dependent on the activation and binding of CSL to the SMA promoter.	bind
23853	3	6472	7	NULL	NULL	NULL	NULL	statement 2	Process		depends on		directly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_12_1468_s_25	16741155	12 Here we demonstrate that Notch-mediated upregulation of SMA is directly dependent on the activation and binding of CSL to the SMA promoter.	bind
23854	4	6472	7	NULL	NULL	NULL	NULL	statement 2	Process		depends on		directly			CSL	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_12_1468_s_25	16741155	12 Here we demonstrate that Notch-mediated upregulation of SMA is directly dependent on the activation and binding of CSL to the SMA promoter.	bind
20252	1	6473	5	NULL	NULL	0	NULL	SRF	NULL		bind	NULL				SMC marker genes	NULL			CArG regions	NULL		0	NULL	NULL	NULL	gw60_circulationres_92_8_856_s_197	12663482	12 However, on RA treatment, cells exhibited a number of histone modifications consistent with chromatin relaxation and SRF bound to CArG regions of SMC marker genes.	bind
20253	2	6473	5	NULL	NULL	0	NULL	histone	NULL	modification of	is consistent with	NULL				chromatin	NULL	relaxation of			NULL		0	NULL	NULL	NULL	gw60_circulationres_92_8_856_s_197	12663482	12 However, on RA treatment, cells exhibited a number of histone modifications consistent with chromatin relaxation and SRF bound to CArG regions of SMC marker genes.	bind
20254	3	6473	5	NULL	NULL	0	NULL	RA	NULL	treatment	exhibit	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_92_8_856_s_197	12663482	12 However, on RA treatment, cells exhibited a number of histone modifications consistent with chromatin relaxation and SRF bound to CArG regions of SMC marker genes.	bind
20255	4	6473	5	NULL	NULL	0	NULL	RA	NULL	treatment	exhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_92_8_856_s_197	12663482	12 However, on RA treatment, cells exhibited a number of histone modifications consistent with chromatin relaxation and SRF bound to CArG regions of SMC marker genes.	bind
23855	1	6473	7	NULL	NULL	NULL	NULL	SRF	GP		bind					SMC marker	GP			CArG regions	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_8_856_s_197	12663482	12 However, on RA treatment, cells exhibited a number of histone modifications consistent with chromatin relaxation and SRF bound to CArG regions of SMC marker genes.	bind
23856	2	6473	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs upon					RA 	Chemical	treatment with			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_8_856_s_197	12663482	12 However, on RA treatment, cells exhibited a number of histone modifications consistent with chromatin relaxation and SRF bound to CArG regions of SMC marker genes.	bind
23857	3	6473	7	NULL	NULL	NULL	NULL	cells	Cell	RA treated	exhibit					histone	GP	modifications of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_8_856_s_197	12663482	12 However, on RA treatment, cells exhibited a number of histone modifications consistent with chromatin relaxation and SRF bound to CArG regions of SMC marker genes.	bind
23858	4	6473	7	NULL	NULL	NULL	NULL	statement 3	Process		is consistent with					chromatin relaxation	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_8_856_s_197	12663482	12 However, on RA treatment, cells exhibited a number of histone modifications consistent with chromatin relaxation and SRF bound to CArG regions of SMC marker genes.	bind
20256	1	6474	5	NULL	NULL	0	NULL	P-selectin	NULL		bind	NULL				PSGL-1	NULL				NULL	on monocytes	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_5_1065_s_25	15705928	12 Importantly, binding of P-selectin to PSGL-1 on monocytes also induces the expression of tissue factor (TF), 2 the main initiator of coagulation in vivo.	bind
20257	2	6474	5	NULL	NULL	0	NULL	statement 1	NULL		induces	NULL				TF	NULL	expression of			NULL	in vivo	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_5_1065_s_25	15705928	12 Importantly, binding of P-selectin to PSGL-1 on monocytes also induces the expression of tissue factor (TF), 2 the main initiator of coagulation in vivo.	bind
20258	3	6474	5	NULL	NULL	0	NULL	TF	NULL		is	NULL				tissue factor	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_5_1065_s_25	15705928	12 Importantly, binding of P-selectin to PSGL-1 on monocytes also induces the expression of tissue factor (TF), 2 the main initiator of coagulation in vivo.	bind
20259	4	6474	5	NULL	NULL	0	NULL	TF	NULL		initiates	NULL				coagulation	NULL				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_5_1065_s_25	15705928	12 Importantly, binding of P-selectin to PSGL-1 on monocytes also induces the expression of tissue factor (TF), 2 the main initiator of coagulation in vivo.	bind
23859	1	6474	7	NULL	NULL	NULL	NULL	P-selectin	GP		bind					PSGL-1	GP				NULL	monocytes	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_5_1065_s_25	15705928	12 Importantly, binding of P-selectin to PSGL-1 on monocytes also induces the expression of tissue factor (TF), 2 the main initiator of coagulation in vivo.	bind
23860	2	6474	7	NULL	NULL	NULL	NULL	statement 1	Process		induce					TF	GP	expression of			NULL	in vivo	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_5_1065_s_25	15705928	12 Importantly, binding of P-selectin to PSGL-1 on monocytes also induces the expression of tissue factor (TF), 2 the main initiator of coagulation in vivo.	bind
23861	3	6474	7	NULL	NULL	NULL	NULL	TF	GP		initiates					coagulation	Process				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_5_1065_s_25	15705928	12 Importantly, binding of P-selectin to PSGL-1 on monocytes also induces the expression of tissue factor (TF), 2 the main initiator of coagulation in vivo.	bind
23862	4	6474	7	NULL	NULL	NULL	NULL	TF	GP		is					Tissue Factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_5_1065_s_25	15705928	12 Importantly, binding of P-selectin to PSGL-1 on monocytes also induces the expression of tissue factor (TF), 2 the main initiator of coagulation in vivo.	bind
20374	1	6475	5	NULL	NULL	0	NULL	mmLDL	NULL		bind	NULL				heat shock protein-60	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1085_s_46	15923538	12 In addition to mmLDL, TLR4 also binds heat shock protein-60, another antigenic protein implicated in atherosclerosis.	bind
20375	2	6475	5	NULL	NULL	0	NULL	TLR4	NULL		bind	NULL				heat shock protein-60	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1085_s_46	15923538	12 In addition to mmLDL, TLR4 also binds heat shock protein-60, another antigenic protein implicated in atherosclerosis.	bind
20376	3	6475	5	NULL	NULL	0	NULL	heat shock protein-60	NULL		is a type of	NULL				antigenic protein	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1085_s_46	15923538	12 In addition to mmLDL, TLR4 also binds heat shock protein-60, another antigenic protein implicated in atherosclerosis.	bind
20377	4	6475	5	NULL	NULL	0	NULL	heat shock protein-60	NULL		is implicated in	NULL				atherosclerosis	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1085_s_46	15923538	12 In addition to mmLDL, TLR4 also binds heat shock protein-60, another antigenic protein implicated in atherosclerosis.	bind
23863	1	6475	7	NULL	NULL	NULL	NULL	TLR4	GP		binds					mmLDL	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1085_s_46	15923538	12 In addition to mmLDL, TLR4 also binds heat shock protein-60, another antigenic protein implicated in atherosclerosis.	bind
23864	2	6475	7	NULL	NULL	NULL	NULL	TLR4	GP		bind					heat shock protein-60	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1085_s_46	15923538	12 In addition to mmLDL, TLR4 also binds heat shock protein-60, another antigenic protein implicated in atherosclerosis.	bind
23865	3	6475	7	NULL	NULL	NULL	NULL	heat shock protein-60	GP		implicated in					atherosclerosis	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1085_s_46	15923538	12 In addition to mmLDL, TLR4 also binds heat shock protein-60, another antigenic protein implicated in atherosclerosis.	bind
30885	4	6475	7	NULL	NULL	NULL	NULL	heat shock protein-60	GP		is a type of					antigenic protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1085_s_46	15923538	12 In addition to mmLDL, TLR4 also binds heat shock protein-60, another antigenic protein implicated in atherosclerosis.	bind
20378	1	6476	5	NULL	NULL	0	NULL	CCL5	NULL		bind	NULL				CCR5 receptor	NULL				NULL		0	NULL	NULL	NULL	gw70_jantimicrobchemoth_53_6_895_s_23	15128728	12 Increased binding of CCL5 to its receptor CCR5 further decreases CCR5 surface density due to receptor internalization.	bind
20380	2	6476	5	NULL	NULL	0	NULL	statement 1	NULL	increased	decreases	NULL				CCR5	NULL	surface density of			NULL		0	NULL	NULL	NULL	gw70_jantimicrobchemoth_53_6_895_s_23	15128728	12 Increased binding of CCL5 to its receptor CCR5 further decreases CCR5 surface density due to receptor internalization.	bind
20381	3	6476	5	NULL	NULL	0	NULL	statement 2	NULL		occurs due to	NULL				receptor internalization	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jantimicrobchemoth_53_6_895_s_23	15128728	12 Increased binding of CCL5 to its receptor CCR5 further decreases CCR5 surface density due to receptor internalization.	bind
23866	1	6476	7	NULL	NULL	NULL	NULL	CCL5	GP		binds to					CCR5 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_jantimicrobchemoth_53_6_895_s_23	15128728	12 Increased binding of CCL5 to its receptor CCR5 further decreases CCR5 surface density due to receptor internalization.	bind
23867	2	6476	7	NULL	NULL	NULL	NULL	statement 1	Process	increased	decrease					CCR5	GP	surface density			NULL		NULL	NULL	NULL	NULL	gw70_jantimicrobchemoth_53_6_895_s_23	15128728	12 Increased binding of CCL5 to its receptor CCR5 further decreases CCR5 surface density due to receptor internalization.	bind
23868	3	6476	7	NULL	NULL	NULL	NULL	statement 2	GP		occurs due to					receptor internalization	Process				NULL		NULL	NULL	NULL	NULL	gw70_jantimicrobchemoth_53_6_895_s_23	15128728	12 Increased binding of CCL5 to its receptor CCR5 further decreases CCR5 surface density due to receptor internalization.	bind
20382	1	6478	5	NULL	NULL	0	NULL	VEGF-C	NULL		undergoes	NULL				proteolytic processing	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_1_11_s_59	9665459	12 Proteolytic processing of VEGF-C generates several VEGF-C forms with increased activity toward VEGFR-3, but only the fully processed VEGF-C can bind to VEGFR-2.	bind
20383	2	6478	5	NULL	NULL	0	NULL	VEGF-C forms	NULL		shows increased activity towards	NULL				VEGFR-3	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_1_11_s_59	9665459	12 Proteolytic processing of VEGF-C generates several VEGF-C forms with increased activity toward VEGFR-3, but only the fully processed VEGF-C can bind to VEGFR-2.	bind
20385	3	6478	5	NULL	NULL	0	NULL	statement 1	NULL		generates	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_1_11_s_59	9665459	12 Proteolytic processing of VEGF-C generates several VEGF-C forms with increased activity toward VEGFR-3, but only the fully processed VEGF-C can bind to VEGFR-2.	bind
20386	4	6478	5	NULL	NULL	0	NULL	VEGF-C	NULL	only fully processed	bind	NULL				VEGFR-2	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_1_11_s_59	9665459	12 Proteolytic processing of VEGF-C generates several VEGF-C forms with increased activity toward VEGFR-3, but only the fully processed VEGF-C can bind to VEGFR-2.	bind
23869	1	6478	7	NULL	NULL	NULL	NULL	VEGF-C	GP	Proteolytic processing of	generates					VEGF-C forms	GP	several			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_1_11_s_59	9665459	12 Proteolytic processing of VEGF-C generates several VEGF-C forms with increased activity toward VEGFR-3, but only the fully processed VEGF-C can bind to VEGFR-2.	bind
23870	2	6478	7	NULL	NULL	NULL	NULL	VEGF-C forms	GP		shows					VEGFR-3	GP	increased activity towards			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_1_11_s_59	9665459	12 Proteolytic processing of VEGF-C generates several VEGF-C forms with increased activity toward VEGFR-3, but only the fully processed VEGF-C can bind to VEGFR-2.	bind
23871	3	6478	7	NULL	NULL	NULL	NULL	VEGF-C	GP	fully processed	bind					VEGFR-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_1_11_s_59	9665459	12 Proteolytic processing of VEGF-C generates several VEGF-C forms with increased activity toward VEGFR-3, but only the fully processed VEGF-C can bind to VEGFR-2.	bind
20384	1	6479	5	NULL	NULL	0	NULL	E1A	NULL		bind	NULL	strongly			importin-alpha3	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_277_41_38755_s_41	12161448	12 S E1A binds strongly to importin-alpha3  in vitro, while Lys239 substitution mutations and acetylation of E1A by CBP abrogate this interaction.	bind
20387	2	6479	5	10	NULL	0	NULL	E1A		substitution mutations	abrogate			Lys239		statement 1					NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_41_38755_s_41	12161448	12 S E1A binds strongly to importin-alpha3  in vitro, while Lys239 substitution mutations and acetylation of E1A by CBP abrogate this interaction.	bind
20388	3	6479	5	NULL	NULL	0	NULL	CBP	NULL		acetylate	NULL				E1A	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_41_38755_s_41	12161448	12 S E1A binds strongly to importin-alpha3  in vitro, while Lys239 substitution mutations and acetylation of E1A by CBP abrogate this interaction.	bind
20389	4	6479	5	10	NULL	0	NULL	statement 3			abrogate					statement 1					NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_41_38755_s_41	12161448	12 S E1A binds strongly to importin-alpha3  in vitro, while Lys239 substitution mutations and acetylation of E1A by CBP abrogate this interaction.	bind
23872	1	6479	7	NULL	NULL	NULL	NULL	S E1A	GP		bind		strongly			importin-alpha3	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_41_38755_s_41	12161448	12 S E1A binds strongly to importin-alpha3  in vitro, while Lys239 substitution mutations and acetylation of E1A by CBP abrogate this interaction.	bind
23873	2	6479	7	NULL	NULL	NULL	NULL	E1A	GP	substitution mutation	abrogates			Lys239		statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_41_38755_s_41	12161448	12 S E1A binds strongly to importin-alpha3  in vitro, while Lys239 substitution mutations and acetylation of E1A by CBP abrogate this interaction.	bind
23874	3	6479	7	NULL	NULL	NULL	NULL	CBP	GP		acetylates					E1A	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_41_38755_s_41	12161448	12 S E1A binds strongly to importin-alpha3  in vitro, while Lys239 substitution mutations and acetylation of E1A by CBP abrogate this interaction.	bind
23875	4	6479	7	NULL	NULL	NULL	NULL	statement 3	Process		abrogates					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_41_38755_s_41	12161448	12 S E1A binds strongly to importin-alpha3  in vitro, while Lys239 substitution mutations and acetylation of E1A by CBP abrogate this interaction.	bind
20390	1	6480	5	NULL	NULL	0	NULL	keratinocytes	NULL	human	is treated with	NULL				arsenic	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_6_1775_s_20	9846968	12 Support exists that increased cell proliferation is a central event, as treatment of human keratinocytes with arsenic induces ornithine decarboxylase activity 13  and growth factor expression 14 as well as alters the DNA-binding activities of the AP-1 and AP-2 transcription factors, which are involved in proliferative events.	bind
20391	2	6480	5	NULL	NULL	0	NULL	statement 1	NULL		induces	NULL				ornithine decarboxylase	NULL	activity of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_6_1775_s_20	9846968	12 Support exists that increased cell proliferation is a central event, as treatment of human keratinocytes with arsenic induces ornithine decarboxylase activity 13  and growth factor expression 14 as well as alters the DNA-binding activities of the AP-1 and AP-2 transcription factors, which are involved in proliferative events.	bind
20392	3	6480	5	NULL	NULL	0	NULL	statement 1	NULL		induces	NULL				growth factor	NULL	expression of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_6_1775_s_20	9846968	12 Support exists that increased cell proliferation is a central event, as treatment of human keratinocytes with arsenic induces ornithine decarboxylase activity 13  and growth factor expression 14 as well as alters the DNA-binding activities of the AP-1 and AP-2 transcription factors, which are involved in proliferative events.	bind
20393	4	6480	5	10	NULL	0	NULL	AP-1	NULL		bind	NULL				DNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_6_1775_s_20	9846968	12 Support exists that increased cell proliferation is a central event, as treatment of human keratinocytes with arsenic induces ornithine decarboxylase activity 13  and growth factor expression 14 as well as alters the DNA-binding activities of the AP-1 and AP-2 transcription factors, which are involved in proliferative events.	bind
20394	5	6480	5	10	NULL	0	NULL	AP-2	NULL		bind	NULL				DNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_6_1775_s_20	9846968	12 Support exists that increased cell proliferation is a central event, as treatment of human keratinocytes with arsenic induces ornithine decarboxylase activity 13  and growth factor expression 14 as well as alters the DNA-binding activities of the AP-1 and AP-2 transcription factors, which are involved in proliferative events.	bind
20395	6	6480	5	NULL	NULL	0	NULL	statement 1	NULL		alters	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_6_1775_s_20	9846968	12 Support exists that increased cell proliferation is a central event, as treatment of human keratinocytes with arsenic induces ornithine decarboxylase activity 13  and growth factor expression 14 as well as alters the DNA-binding activities of the AP-1 and AP-2 transcription factors, which are involved in proliferative events.	bind
20396	7	6480	5	NULL	NULL	0	NULL	statement 1	NULL		alters	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_6_1775_s_20	9846968	12 Support exists that increased cell proliferation is a central event, as treatment of human keratinocytes with arsenic induces ornithine decarboxylase activity 13  and growth factor expression 14 as well as alters the DNA-binding activities of the AP-1 and AP-2 transcription factors, which are involved in proliferative events.	bind
20397	8	6480	5	10	NULL	0	NULL	AP-1	NULL		is involved in	NULL				proliferative events	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_6_1775_s_20	9846968	12 Support exists that increased cell proliferation is a central event, as treatment of human keratinocytes with arsenic induces ornithine decarboxylase activity 13  and growth factor expression 14 as well as alters the DNA-binding activities of the AP-1 and AP-2 transcription factors, which are involved in proliferative events.	bind
20398	9	6480	5	10	NULL	0	NULL	AP-2	NULL		is involved in	NULL				proliferative events	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_6_1775_s_20	9846968	12 Support exists that increased cell proliferation is a central event, as treatment of human keratinocytes with arsenic induces ornithine decarboxylase activity 13  and growth factor expression 14 as well as alters the DNA-binding activities of the AP-1 and AP-2 transcription factors, which are involved in proliferative events.	bind
45624	10	6480	5	10	NULL	0	NULL	AP1	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_6_1775_s_20	9846968	12 Support exists that increased cell proliferation is a central event, as treatment of human keratinocytes with arsenic induces ornithine decarboxylase activity 13  and growth factor expression 14 as well as alters the DNA-binding activities of the AP-1 and AP-2 transcription factors, which are involved in proliferative events.	bind
45625	11	6480	5	10	NULL	0	NULL	AP2	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_6_1775_s_20	9846968	12 Support exists that increased cell proliferation is a central event, as treatment of human keratinocytes with arsenic induces ornithine decarboxylase activity 13  and growth factor expression 14 as well as alters the DNA-binding activities of the AP-1 and AP-2 transcription factors, which are involved in proliferative events.	bind
23876	1	6480	7	NULL	NULL	NULL	NULL	keratinocytes	Cell	arsenic treated;;human	induce					ornithine decarboxylase	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_6_1775_s_20	9846968	12 Support exists that increased cell proliferation is a central event, as treatment of human keratinocytes with arsenic induces ornithine decarboxylase activity 13  and growth factor expression 14 as well as alters the DNA-binding activities of the AP-1 and AP-2 transcription factors, which are involved in proliferative events.	bind
23877	2	6480	7	NULL	NULL	NULL	NULL	keratinocytes	Cell	arsenic treated;;human	induce					growth factor	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_6_1775_s_20	9846968	12 Support exists that increased cell proliferation is a central event, as treatment of human keratinocytes with arsenic induces ornithine decarboxylase activity 13  and growth factor expression 14 as well as alters the DNA-binding activities of the AP-1 and AP-2 transcription factors, which are involved in proliferative events.	bind
23878	3	6480	7	NULL	NULL	NULL	NULL	AP-1	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_6_1775_s_20	9846968	12 Support exists that increased cell proliferation is a central event, as treatment of human keratinocytes with arsenic induces ornithine decarboxylase activity 13  and growth factor expression 14 as well as alters the DNA-binding activities of the AP-1 and AP-2 transcription factors, which are involved in proliferative events.	bind
23879	4	6480	7	NULL	NULL	NULL	NULL	AP-2	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_6_1775_s_20	9846968	12 Support exists that increased cell proliferation is a central event, as treatment of human keratinocytes with arsenic induces ornithine decarboxylase activity 13  and growth factor expression 14 as well as alters the DNA-binding activities of the AP-1 and AP-2 transcription factors, which are involved in proliferative events.	bind
23880	5	6480	7	NULL	NULL	NULL	NULL	keratinocytes	Cell	arsenic treated;;human	increase					cell proliferation	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_6_1775_s_20	9846968	12 Support exists that increased cell proliferation is a central event, as treatment of human keratinocytes with arsenic induces ornithine decarboxylase activity 13  and growth factor expression 14 as well as alters the DNA-binding activities of the AP-1 and AP-2 transcription factors, which are involved in proliferative events.	bind
23881	6	6480	7	NULL	NULL	NULL	NULL	keratinocytes	Cell	arsenic treated;;human	alters					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_6_1775_s_20	9846968	12 Support exists that increased cell proliferation is a central event, as treatment of human keratinocytes with arsenic induces ornithine decarboxylase activity 13  and growth factor expression 14 as well as alters the DNA-binding activities of the AP-1 and AP-2 transcription factors, which are involved in proliferative events.	bind
23882	7	6480	7	NULL	NULL	NULL	NULL	keratinocytes	Cell	arsenic treated;;human	alters					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_6_1775_s_20	9846968	12 Support exists that increased cell proliferation is a central event, as treatment of human keratinocytes with arsenic induces ornithine decarboxylase activity 13  and growth factor expression 14 as well as alters the DNA-binding activities of the AP-1 and AP-2 transcription factors, which are involved in proliferative events.	bind
23887	8	6480	7	NULL	NULL	NULL	NULL	AP-1	GP		is involved in					proliferative events	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_6_1775_s_20	9846968	12 Support exists that increased cell proliferation is a central event, as treatment of human keratinocytes with arsenic induces ornithine decarboxylase activity 13  and growth factor expression 14 as well as alters the DNA-binding activities of the AP-1 and AP-2 transcription factors, which are involved in proliferative events.	bind
23888	9	6480	7	NULL	NULL	NULL	NULL	AP-2	GP		is involved in					proliferative events	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_6_1775_s_20	9846968	12 Support exists that increased cell proliferation is a central event, as treatment of human keratinocytes with arsenic induces ornithine decarboxylase activity 13  and growth factor expression 14 as well as alters the DNA-binding activities of the AP-1 and AP-2 transcription factors, which are involved in proliferative events.	bind
45626	10	6480	7	NULL	NULL	NULL	NULL	AP1	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_6_1775_s_20	9846968	12 Support exists that increased cell proliferation is a central event, as treatment of human keratinocytes with arsenic induces ornithine decarboxylase activity 13  and growth factor expression 14 as well as alters the DNA-binding activities of the AP-1 and AP-2 transcription factors, which are involved in proliferative events.	bind
45627	11	6480	7	NULL	NULL	NULL	NULL	AP2	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_6_1775_s_20	9846968	12 Support exists that increased cell proliferation is a central event, as treatment of human keratinocytes with arsenic induces ornithine decarboxylase activity 13  and growth factor expression 14 as well as alters the DNA-binding activities of the AP-1 and AP-2 transcription factors, which are involved in proliferative events.	bind
20399	1	6481	5	NULL	NULL	0	NULL	CV-N	NULL		is	NULL				cyanovirin-N	NULL				NULL		0	NULL	NULL	NULL	gw70_jantimicrobchemoth_52_6_890_s_74	14613946	12 The cyanobacterial protein cyanovirin-N (CV-N) binds to gp120 via mannose moieties on individual N-linked glycans.	bind
20400	2	6481	5	NULL	NULL	0	NULL	CV-N	NULL	cyanobacterial protein	bind	NULL				gp120	NULL				NULL		0	NULL	NULL	NULL	gw70_jantimicrobchemoth_52_6_890_s_74	14613946	12 The cyanobacterial protein cyanovirin-N (CV-N) binds to gp120 via mannose moieties on individual N-linked glycans.	bind
20401	3	6481	5	NULL	NULL	0	NULL	statement 2	NULL		via	NULL				N-linked glycans	NULL	individual	mannose moieties		NULL		NULL	NULL	NULL	NULL	gw70_jantimicrobchemoth_52_6_890_s_74	14613946	12 The cyanobacterial protein cyanovirin-N (CV-N) binds to gp120 via mannose moieties on individual N-linked glycans.	bind
23889	1	6481	7	NULL	NULL	NULL	NULL	CV-N	GP	cyanobacterial protein	binds to					gp120	Gp				NULL		NULL	NULL	NULL	NULL	gw70_jantimicrobchemoth_52_6_890_s_74	14613946	12 The cyanobacterial protein cyanovirin-N (CV-N) binds to gp120 via mannose moieties on individual N-linked glycans.	bind
23890	2	6481	7	NULL	NULL	NULL	NULL	statement 1	Process		 via					N-linked glycans	Chemical		mannose moieties		NULL		NULL	NULL	NULL	NULL	gw70_jantimicrobchemoth_52_6_890_s_74	14613946	12 The cyanobacterial protein cyanovirin-N (CV-N) binds to gp120 via mannose moieties on individual N-linked glycans.	bind
23891	3	6481	7	NULL	NULL	NULL	NULL	CV-N	GP		is					cyanovirin-N	GP				NULL		NULL	NULL	NULL	NULL	gw70_jantimicrobchemoth_52_6_890_s_74	14613946	12 The cyanobacterial protein cyanovirin-N (CV-N) binds to gp120 via mannose moieties on individual N-linked glycans.	bind
20402	1	6483	5	NULL	NULL	0	NULL	IAP	NULL		bind	NULL				SHPS-1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_93_10_925_s_202	14563713	12 We have shown recently that when IAP binding to SHPS-1 is blocked, IGF-I - stimulated SHPS-1 phosphorylation is inhibited.	bind
20403	2	6483	5	NULL	NULL	0	NULL	IGF-I	NULL		stimulates	NULL				SHPS-1	NULL	phosphorylation of			NULL		0	NULL	NULL	NULL	gw70_circulationres_93_10_925_s_202	14563713	12 We have shown recently that when IAP binding to SHPS-1 is blocked, IGF-I - stimulated SHPS-1 phosphorylation is inhibited.	bind
20404	3	6483	5	NULL	NULL	0	NULL	statement 1	NULL	blocking of	leads to	NULL				statement 2	NULL	inhibition of			NULL		0	NULL	NULL	NULL	gw70_circulationres_93_10_925_s_202	14563713	12 We have shown recently that when IAP binding to SHPS-1 is blocked, IGF-I - stimulated SHPS-1 phosphorylation is inhibited.	bind
23892	1	6483	7	NULL	NULL	NULL	NULL	IAP 	GP		bind					SHPS-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_10_925_s_202	14563713	12 We have shown recently that when IAP binding to SHPS-1 is blocked, IGF-I - stimulated SHPS-1 phosphorylation is inhibited.	bind
23893	2	6483	7	NULL	NULL	NULL	NULL	IGF-I 	GP		stimulates					SHPS-1	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_10_925_s_202	14563713	12 We have shown recently that when IAP binding to SHPS-1 is blocked, IGF-I - stimulated SHPS-1 phosphorylation is inhibited.	bind
23894	3	6483	7	NULL	NULL	NULL	NULL	statement 1	Process	blocking	results in					statement 2	Process	inhibition of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_10_925_s_202	14563713	12 We have shown recently that when IAP binding to SHPS-1 is blocked, IGF-I - stimulated SHPS-1 phosphorylation is inhibited.	bind
20405	1	6485	5	NULL	NULL	0	NULL	PlA2 variant platelet	NULL		bind	NULL				fibrinogen	NULL	exogenous			NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_2_140_s_32	11447076	12, 13 Paradoxically, however, Goldschmidt-Clermont et al 14 showed that platelets with the  PlA2 variant bound less exogenous fibrinogen than did the  PlA1-homozygous platelets when stimulated with ADP.	bind
20406	2	6485	5	NULL	NULL	0	NULL	PlA1-homozygous platelets	NULL		bind	NULL				fibrinogen	NULL	exogenous			NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_2_140_s_32	11447076	12, 13 Paradoxically, however, Goldschmidt-Clermont et al 14 showed that platelets with the  PlA2 variant bound less exogenous fibrinogen than did the  PlA1-homozygous platelets when stimulated with ADP.	bind
20407	3	6485	5	NULL	NULL	0	NULL	statement 1	NULL		is lesser than	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_104_2_140_s_32	11447076	12, 13 Paradoxically, however, Goldschmidt-Clermont et al 14 showed that platelets with the  PlA2 variant bound less exogenous fibrinogen than did the  PlA1-homozygous platelets when stimulated with ADP.	bind
20408	4	6485	5	NULL	NULL	0	NULL	statement 3	NULL		occurs on	NULL				ADP	NULL	stimulation with			NULL		0	NULL	NULL	NULL	gw60_circulation_104_2_140_s_32	11447076	12, 13 Paradoxically, however, Goldschmidt-Clermont et al 14 showed that platelets with the  PlA2 variant bound less exogenous fibrinogen than did the  PlA1-homozygous platelets when stimulated with ADP.	bind
23895	1	6485	7	NULL	NULL	NULL	NULL	PlA2 variant platelet	Cell		bind					fibrinogen	GP	exogenous			NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_2_140_s_32	11447076	12, 13 Paradoxically, however, Goldschmidt-Clermont et al 14 showed that platelets with the  PlA2 variant bound less exogenous fibrinogen than did the  PlA1-homozygous platelets when stimulated with ADP.	bind
23896	2	6485	7	NULL	NULL	NULL	NULL	PlA1-homozygous platelets	Cell		bind					fibrinogen	GP	exogenous			NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_2_140_s_32	11447076	12, 13 Paradoxically, however, Goldschmidt-Clermont et al 14 showed that platelets with the  PlA2 variant bound less exogenous fibrinogen than did the  PlA1-homozygous platelets when stimulated with ADP.	bind
23897	3	6485	7	NULL	NULL	NULL	NULL	statement 1	Process	binding of	is less than					statement 2	Process	binding of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_2_140_s_32	11447076	12, 13 Paradoxically, however, Goldschmidt-Clermont et al 14 showed that platelets with the  PlA2 variant bound less exogenous fibrinogen than did the  PlA1-homozygous platelets when stimulated with ADP.	bind
23898	4	6485	7	NULL	NULL	NULL	NULL	statement 3	Process		occurs when					ADP	Chemical	stimulated with			NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_2_140_s_32	11447076	12, 13 Paradoxically, however, Goldschmidt-Clermont et al 14 showed that platelets with the  PlA2 variant bound less exogenous fibrinogen than did the  PlA1-homozygous platelets when stimulated with ADP.	bind
20409	1	6486	5	10	NULL	0	NULL	ets			bind			DNA-binding domain						GGA(A/T) DNA sequence	NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_10_1411_s_31	12642363	12, 13 The ets family of transcription factors has a common DNA-binding domain that binds to a core GGA(A/T) DNA sequence.	bind
54268	2	6486	5	10	NULL	0	NULL	ets			is a type of					transcription factor					NULL		0	NULL	NULL	NULL	gw60_circulation_107_10_1411_s_31	12642363	12, 13 The ets family of transcription factors has a common DNA-binding domain that binds to a core GGA(A/T) DNA sequence.	bind
24058	1	6486	7	NULL	NULL	NULL	NULL	ets	GP		binds			DNA-binding domain						core GGA(A/T) DNA sequence	NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_10_1411_s_31	12642363	12, 13 The ets family of transcription factors has a common DNA-binding domain that binds to a core GGA(A/T) DNA sequence.	bind
30886	2	6486	7	NULL	NULL	NULL	NULL	ets	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_10_1411_s_31	12642363	12, 13 The ets family of transcription factors has a common DNA-binding domain that binds to a core GGA(A/T) DNA sequence.	bind
20411	1	6488	5	NULL	NULL	0	NULL	LRR	NULL		bind	NULL			cis-regulatory element	NF-kappaB	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_162	12600889	12, 19 The LRR contains the  cis-regulatory element for NF-kappaB and AP-1 binding on stimulation by inflammatory mediators such as LPS, TNF-alpha, or IL-1beta.	bind
20412	2	6488	5	NULL	NULL	0	NULL	LRR	NULL		bind	NULL			cis-regulatory element	AP-1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_162	12600889	12, 19 The LRR contains the  cis-regulatory element for NF-kappaB and AP-1 binding on stimulation by inflammatory mediators such as LPS, TNF-alpha, or IL-1beta.	bind
20413	3	6488	5	NULL	NULL	0	NULL	LPS	NULL		stimulates	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_162	12600889	12, 19 The LRR contains the  cis-regulatory element for NF-kappaB and AP-1 binding on stimulation by inflammatory mediators such as LPS, TNF-alpha, or IL-1beta.	bind
20414	4	6488	5	NULL	NULL	0	NULL	LPS	NULL		stimulates	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_162	12600889	12, 19 The LRR contains the  cis-regulatory element for NF-kappaB and AP-1 binding on stimulation by inflammatory mediators such as LPS, TNF-alpha, or IL-1beta.	bind
20415	5	6488	5	NULL	NULL	0	NULL	TNF-alpha	NULL		stimulates	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_162	12600889	12, 19 The LRR contains the  cis-regulatory element for NF-kappaB and AP-1 binding on stimulation by inflammatory mediators such as LPS, TNF-alpha, or IL-1beta.	bind
20416	6	6488	5	NULL	NULL	0	NULL	TNF-alpha	NULL		stimulates	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_162	12600889	12, 19 The LRR contains the  cis-regulatory element for NF-kappaB and AP-1 binding on stimulation by inflammatory mediators such as LPS, TNF-alpha, or IL-1beta.	bind
20417	7	6488	5	NULL	NULL	0	NULL	IL-1beta	NULL		stimulates	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_162	12600889	12, 19 The LRR contains the  cis-regulatory element for NF-kappaB and AP-1 binding on stimulation by inflammatory mediators such as LPS, TNF-alpha, or IL-1beta.	bind
20418	8	6488	5	NULL	NULL	0	NULL	IL-1beta	NULL		stimulates	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_162	12600889	12, 19 The LRR contains the  cis-regulatory element for NF-kappaB and AP-1 binding on stimulation by inflammatory mediators such as LPS, TNF-alpha, or IL-1beta.	bind
30264	9	6488	5	NULL	NULL	0	NULL	LPS	NULL		is a type of	NULL				inflammatory mediator	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_162	12600889	12, 19 The LRR contains the  cis-regulatory element for NF-kappaB and AP-1 binding on stimulation by inflammatory mediators such as LPS, TNF-alpha, or IL-1beta.	bind
30265	10	6488	5	NULL	NULL	0	NULL	TNF-alpha	NULL		is a type of	NULL				inflammatory mediator	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_162	12600889	12, 19 The LRR contains the  cis-regulatory element for NF-kappaB and AP-1 binding on stimulation by inflammatory mediators such as LPS, TNF-alpha, or IL-1beta.	bind
30266	11	6488	5	NULL	NULL	0	NULL	IL-1beta	NULL		is a type of	NULL				inflammatory mediator	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_162	12600889	12, 19 The LRR contains the  cis-regulatory element for NF-kappaB and AP-1 binding on stimulation by inflammatory mediators such as LPS, TNF-alpha, or IL-1beta.	bind
24069	1	6488	7	NULL	NULL	NULL	NULL	LRR	GP		bind				cis-regulatory element 	NF-kappaB	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_162	12600889	12, 19 The LRR contains the  cis-regulatory element for NF-kappaB and AP-1 binding on stimulation by inflammatory mediators such as LPS, TNF-alpha, or IL-1beta.	bind
24071	2	6488	7	NULL	NULL	NULL	NULL	LRR	GP		bind				cis-regulatory element 	AP-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_162	12600889	12, 19 The LRR contains the  cis-regulatory element for NF-kappaB and AP-1 binding on stimulation by inflammatory mediators such as LPS, TNF-alpha, or IL-1beta.	bind
24073	3	6488	7	NULL	NULL	NULL	NULL	LPS	Chemical		stimulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_162	12600889	12, 19 The LRR contains the  cis-regulatory element for NF-kappaB and AP-1 binding on stimulation by inflammatory mediators such as LPS, TNF-alpha, or IL-1beta.	bind
24074	4	6488	7	NULL	NULL	NULL	NULL	TNF-alpha	GP		stimulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_162	12600889	12, 19 The LRR contains the  cis-regulatory element for NF-kappaB and AP-1 binding on stimulation by inflammatory mediators such as LPS, TNF-alpha, or IL-1beta.	bind
24078	5	6488	7	NULL	NULL	NULL	NULL	IL-1beta	GP		stimulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_162	12600889	12, 19 The LRR contains the  cis-regulatory element for NF-kappaB and AP-1 binding on stimulation by inflammatory mediators such as LPS, TNF-alpha, or IL-1beta.	bind
24079	6	6488	7	NULL	NULL	NULL	NULL	LPS	Chemical		stimulates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_162	12600889	12, 19 The LRR contains the  cis-regulatory element for NF-kappaB and AP-1 binding on stimulation by inflammatory mediators such as LPS, TNF-alpha, or IL-1beta.	bind
24080	7	6488	7	NULL	NULL	NULL	NULL	TNF-alpha	GP		stimulates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_162	12600889	12, 19 The LRR contains the  cis-regulatory element for NF-kappaB and AP-1 binding on stimulation by inflammatory mediators such as LPS, TNF-alpha, or IL-1beta.	bind
24081	8	6488	7	NULL	NULL	NULL	NULL	IL-1beta	GP		stimulates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_162	12600889	12, 19 The LRR contains the  cis-regulatory element for NF-kappaB and AP-1 binding on stimulation by inflammatory mediators such as LPS, TNF-alpha, or IL-1beta.	bind
30887	9	6488	7	NULL	NULL	NULL	NULL	LPS	Chemical		is a type of					inflammatory mediator	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_162	12600889	12, 19 The LRR contains the  cis-regulatory element for NF-kappaB and AP-1 binding on stimulation by inflammatory mediators such as LPS, TNF-alpha, or IL-1beta.	bind
30888	10	6488	7	NULL	NULL	NULL	NULL	TNF-alpha	GP		is a type of					inflammatory mediator	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_162	12600889	12, 19 The LRR contains the  cis-regulatory element for NF-kappaB and AP-1 binding on stimulation by inflammatory mediators such as LPS, TNF-alpha, or IL-1beta.	bind
30889	11	6488	7	NULL	NULL	NULL	NULL	IL-1beta	GP		is a type of					inflammatory mediator	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_162	12600889	12, 19 The LRR contains the  cis-regulatory element for NF-kappaB and AP-1 binding on stimulation by inflammatory mediators such as LPS, TNF-alpha, or IL-1beta.	bind
20419	1	6489	5	NULL	NULL	0	NULL	VEGF	NULL		bind	NULL				heparin	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_1_11_s_56	9665459	12, 35, 36  Unlike some of the VEGF, VEGF-B, and PlGF isoforms, VEGF-C does not bind to heparin.	bind
20420	2	6489	5	NULL	NULL	0	NULL	VEGF-B	NULL		bind	NULL				heparin	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_1_11_s_56	9665459	12, 35, 36  Unlike some of the VEGF, VEGF-B, and PlGF isoforms, VEGF-C does not bind to heparin.	bind
20421	3	6489	5	NULL	NULL	0	NULL	PlGF isoforms	NULL		bind	NULL				heparin	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_1_11_s_56	9665459	12, 35, 36  Unlike some of the VEGF, VEGF-B, and PlGF isoforms, VEGF-C does not bind to heparin.	bind
20422	4	6489	5	NULL	NULL	0	NULL	VEGF-C	NULL		does not bind	NULL				heparin	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_1_11_s_56	9665459	12, 35, 36  Unlike some of the VEGF, VEGF-B, and PlGF isoforms, VEGF-C does not bind to heparin.	bind
24082	1	6489	7	NULL	NULL	NULL	NULL	VEGF-C	GP		does not bind					heparin	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_1_11_s_56	9665459	12, 35, 36  Unlike some of the VEGF, VEGF-B, and PlGF isoforms, VEGF-C does not bind to heparin.	bind
24083	2	6489	7	NULL	NULL	NULL	NULL	VEGF	GP		bind					heparin	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_1_11_s_56	9665459	12, 35, 36  Unlike some of the VEGF, VEGF-B, and PlGF isoforms, VEGF-C does not bind to heparin.	bind
24084	3	6489	7	NULL	NULL	NULL	NULL	VEGF-B	GP		bind					heparin	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_1_11_s_56	9665459	12, 35, 36  Unlike some of the VEGF, VEGF-B, and PlGF isoforms, VEGF-C does not bind to heparin.	bind
24085	4	6489	7	NULL	NULL	NULL	NULL	PlGF isoform	GP		bind					heparin	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_1_11_s_56	9665459	12, 35, 36  Unlike some of the VEGF, VEGF-B, and PlGF isoforms, VEGF-C does not bind to heparin.	bind
20423	1	6490	5	NULL	NULL	0	NULL	CRP	NULL		bind	NULL				LDL	NULL	oxidized			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_30	15692104	12,13  In addition, binding of CRP to oxidized LDL and degraded nonoxidized LDL transforms the acute-phase protein to an activator of the classical complement pathway.	bind
20424	2	6490	5	10	NULL	0	NULL	CRP	NULL		bind	NULL				LDL	NULL	degraded;; nonoxidized			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_30	15692104	12,13  In addition, binding of CRP to oxidized LDL and degraded nonoxidized LDL transforms the acute-phase protein to an activator of the classical complement pathway.	bind
20425	3	6490	5	NULL	NULL	0	NULL	acute-phase protein	NULL		is transformed to	NULL				classical complement pathway activator	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_30	15692104	12,13  In addition, binding of CRP to oxidized LDL and degraded nonoxidized LDL transforms the acute-phase protein to an activator of the classical complement pathway.	bind
20426	4	6490	5	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_30	15692104	12,13  In addition, binding of CRP to oxidized LDL and degraded nonoxidized LDL transforms the acute-phase protein to an activator of the classical complement pathway.	bind
20427	5	6490	5	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_30	15692104	12,13  In addition, binding of CRP to oxidized LDL and degraded nonoxidized LDL transforms the acute-phase protein to an activator of the classical complement pathway.	bind
24086	1	6490	7	NULL	NULL	NULL	NULL	CRP 	GP		bind					 LDL	GP	oxidized			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_30	15692104	12,13  In addition, binding of CRP to oxidized LDL and degraded nonoxidized LDL transforms the acute-phase protein to an activator of the classical complement pathway.	bind
24087	2	6490	7	NULL	NULL	NULL	NULL	CRP	GP		bind					LDL	GP	degraded;; nonoxidized			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_30	15692104	12,13  In addition, binding of CRP to oxidized LDL and degraded nonoxidized LDL transforms the acute-phase protein to an activator of the classical complement pathway.	bind
24088	3	6490	7	NULL	NULL	NULL	NULL	acute-phase protein	GP		become an					classical complement pathway activator	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_30	15692104	12,13  In addition, binding of CRP to oxidized LDL and degraded nonoxidized LDL transforms the acute-phase protein to an activator of the classical complement pathway.	bind
24089	4	6490	7	NULL	NULL	NULL	NULL	statement 1	Process		transform					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_30	15692104	12,13  In addition, binding of CRP to oxidized LDL and degraded nonoxidized LDL transforms the acute-phase protein to an activator of the classical complement pathway.	bind
24090	5	6490	7	NULL	NULL	NULL	NULL	statement 2	Process		transform					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_30	15692104	12,13  In addition, binding of CRP to oxidized LDL and degraded nonoxidized LDL transforms the acute-phase protein to an activator of the classical complement pathway.	bind
20428	1	6491	5	NULL	NULL	0	NULL	agonists	NULL		bind	NULL				G-protein - coupled receptors	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_93_7_630_s_26	12946946	12,13  Such agonists that bind to G-protein - coupled receptors produced contraction by increasing both the cytosolic Ca2+ concentration and the Ca2+ sensitivity of the contractile apparatus.	bind
20429	2	6491	5	NULL	NULL	0	NULL	statement 1	NULL		produces	NULL				contraction	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_93_7_630_s_26	12946946	12,13  Such agonists that bind to G-protein - coupled receptors produced contraction by increasing both the cytosolic Ca2+ concentration and the Ca2+ sensitivity of the contractile apparatus.	bind
20430	3	6491	5	NULL	NULL	0	NULL	Ca2+ 	NULL	increased cytosolic concentration of	leads to	NULL				statement 2	NULL				NULL	contractile apparatus	0	NULL	NULL	NULL	gw70_circulationres_93_7_630_s_26	12946946	12,13  Such agonists that bind to G-protein - coupled receptors produced contraction by increasing both the cytosolic Ca2+ concentration and the Ca2+ sensitivity of the contractile apparatus.	bind
20431	4	6491	5	NULL	NULL	0	NULL	Ca2+	NULL	increased sensitivity of	leads to	NULL				statement 2	NULL				NULL	contractile apparatus	NULL	NULL	NULL	NULL	gw70_circulationres_93_7_630_s_26	12946946	12,13  Such agonists that bind to G-protein - coupled receptors produced contraction by increasing both the cytosolic Ca2+ concentration and the Ca2+ sensitivity of the contractile apparatus.	bind
24091	2	6491	7	NULL	NULL	NULL	NULL	statement 1	Process		produce					contraction	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_7_630_s_26	12946946	12,13  Such agonists that bind to G-protein - coupled receptors produced contraction by increasing both the cytosolic Ca2+ concentration and the Ca2+ sensitivity of the contractile apparatus.	bind
24092	3	6491	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs by					Ca2+	Chemical	increased cytosolic concentration of 			NULL	contractile appartus	NULL	NULL	NULL	NULL	gw70_circulationres_93_7_630_s_26	12946946	12,13  Such agonists that bind to G-protein - coupled receptors produced contraction by increasing both the cytosolic Ca2+ concentration and the Ca2+ sensitivity of the contractile apparatus.	bind
24093	4	6491	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs by					Ca2+	Chemical	increased sensitivity of 			NULL	contractile appartus	NULL	NULL	NULL	NULL	gw70_circulationres_93_7_630_s_26	12946946	12,13  Such agonists that bind to G-protein - coupled receptors produced contraction by increasing both the cytosolic Ca2+ concentration and the Ca2+ sensitivity of the contractile apparatus.	bind
30901	1	6491	7	NULL	NULL	NULL	NULL	agonists	GP		bind					G-protein-coupled receptors	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_7_630_s_26	12946946	12,13  Such agonists that bind to G-protein - coupled receptors produced contraction by increasing both the cytosolic Ca2+ concentration and the Ca2+ sensitivity of the contractile apparatus.	bind
20432	1	6492	5	NULL	NULL	0	NULL	FVII	NULL		bind	NULL	probably			TF	NULL	extravascular			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_41_s_66	16254201	12,13  Thus, FVII is probably bound to extravascular TF even in the absence of an injury, and the extravascular factors X and IX can be activated as they pass through the tissues.	bind
20433	2	6492	5	NULL	NULL	0	NULL	statement 1	NULL		in the absence of	NULL				injury	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_41_s_66	16254201	12,13  Thus, FVII is probably bound to extravascular TF even in the absence of an injury, and the extravascular factors X and IX can be activated as they pass through the tissues.	bind
20434	3	6492	5	10	NULL	0	NULL	extravascular factor X			pass through					tissues					NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_41_s_66	16254201	12,13  Thus, FVII is probably bound to extravascular TF even in the absence of an injury, and the extravascular factors X and IX can be activated as they pass through the tissues.	bind
20435	4	6492	5	10	NULL	0	NULL	extravascular factor IX			pass through					tissues					NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_41_s_66	16254201	12,13  Thus, FVII is probably bound to extravascular TF even in the absence of an injury, and the extravascular factors X and IX can be activated as they pass through the tissues.	bind
54269	5	6492	5	10	NULL	0	NULL	statement 3			activates					extravascular factors X					NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_41_s_66	16254201	12,13  Thus, FVII is probably bound to extravascular TF even in the absence of an injury, and the extravascular factors X and IX can be activated as they pass through the tissues.	bind
54270	6	6492	5	10	NULL	0	NULL	statement 4			activates					extravascular factors IX					NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_41_s_66	16254201	12,13  Thus, FVII is probably bound to extravascular TF even in the absence of an injury, and the extravascular factors X and IX can be activated as they pass through the tissues.	bind
24094	1	6492	7	NULL	NULL	NULL	NULL	FVII 	GP		bind		probably			TF	GP	extravascular			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_41_s_66	16254201	12,13  Thus, FVII is probably bound to extravascular TF even in the absence of an injury, and the extravascular factors X and IX can be activated as they pass through the tissues.	bind
24095	2	6492	7	NULL	NULL	NULL	NULL	statement 1	Process		in absence of					injury	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_41_s_66	16254201	12,13  Thus, FVII is probably bound to extravascular TF even in the absence of an injury, and the extravascular factors X and IX can be activated as they pass through the tissues.	bind
24096	3	6492	7	NULL	NULL	NULL	NULL	extravascular factor X	GP		pass through					tissues	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_41_s_66	16254201	12,13  Thus, FVII is probably bound to extravascular TF even in the absence of an injury, and the extravascular factors X and IX can be activated as they pass through the tissues.	bind
24097	4	6492	7	NULL	NULL	NULL	NULL	extravascular factor IX	GP		pass through					tissues	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_41_s_66	16254201	12,13  Thus, FVII is probably bound to extravascular TF even in the absence of an injury, and the extravascular factors X and IX can be activated as they pass through the tissues.	bind
54271	5	6492	7	NULL	NULL	NULL	NULL	statement 3	Process		activates					extravascular factors X	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_41_s_66	16254201	12,13  Thus, FVII is probably bound to extravascular TF even in the absence of an injury, and the extravascular factors X and IX can be activated as they pass through the tissues.	bind
54272	6	6492	7	NULL	NULL	NULL	NULL	statement 4	Process		activates					extravascular factors IX	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_41_s_66	16254201	12,13  Thus, FVII is probably bound to extravascular TF even in the absence of an injury, and the extravascular factors X and IX can be activated as they pass through the tissues.	bind
20436	1	6494	5	NULL	NULL	0	NULL	AP-1	NULL		bind	NULL				sPLA2-IIA	NULL	rat		promoter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_27_25830_s_196	15878884	12/15-LOX Enhances Binding of AP-1 to Rat sPLA2-IIA Promoter --	bind
20437	2	6494	5	NULL	NULL	0	NULL	LOX	NULL		enhances	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_27_25830_s_196	15878884	12/15-LOX Enhances Binding of AP-1 to Rat sPLA2-IIA Promoter --	bind
24098	1	6494	7	NULL	NULL	NULL	NULL	AP-1	GP		bind					sPLA2-IIA 	GP	rat		promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_27_25830_s_196	15878884	12/15-LOX Enhances Binding of AP-1 to Rat sPLA2-IIA Promoter --	bind
24099	2	6494	7	NULL	NULL	NULL	NULL	12/15-LOX	GP		enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_27_25830_s_196	15878884	12/15-LOX Enhances Binding of AP-1 to Rat sPLA2-IIA Promoter --	bind
20438	1	6495	5	10	NULL	0	NULL	Bcl-xL	NULL	mutant	is defective for	NULL				Bax	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_154	15539639	120 Consistent with this model, a Bcl-xL mutant, which is defective for Bax and Bak binding but competent to bind tBid, is still cytoprotective.	bind
20439	2	6495	5	NULL	NULL	0	NULL	Bcl-xL	NULL	mutant	is defective for	NULL				Bak	NULL	binding of			NULL		0	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_154	15539639	120 Consistent with this model, a Bcl-xL mutant, which is defective for Bax and Bak binding but competent to bind tBid, is still cytoprotective.	bind
20440	3	6495	5	10	NULL	0	NULL	Bcl-xL		mutant	bind					tBid					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_154	15539639	120 Consistent with this model, a Bcl-xL mutant, which is defective for Bax and Bak binding but competent to bind tBid, is still cytoprotective.	bind
20441	4	6495	5	NULL	NULL	0	NULL	cytoprotective	NULL		is a characteristic of	NULL				Bcl-xL	NULL	mutant			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_154	15539639	120 Consistent with this model, a Bcl-xL mutant, which is defective for Bax and Bak binding but competent to bind tBid, is still cytoprotective.	bind
24100	1	6495	7	NULL	NULL	NULL	NULL	Bcl-xL	GP	mutant	defective in 					Bax	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_154	15539639	120 Consistent with this model, a Bcl-xL mutant, which is defective for Bax and Bak binding but competent to bind tBid, is still cytoprotective.	bind
24101	2	6495	7	NULL	NULL	NULL	NULL	Bcl-xL	GP	mutant	defective in 					Bak	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_154	15539639	120 Consistent with this model, a Bcl-xL mutant, which is defective for Bax and Bak binding but competent to bind tBid, is still cytoprotective.	bind
24102	3	6495	7	NULL	NULL	NULL	NULL	Bcl-xL	GP	mutant	bind					tBid	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_154	15539639	120 Consistent with this model, a Bcl-xL mutant, which is defective for Bax and Bak binding but competent to bind tBid, is still cytoprotective.	bind
24103	4	6495	7	NULL	NULL	NULL	NULL	cytoprotective	Process		is a characteristic of					Bcl-xL	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_154	15539639	120 Consistent with this model, a Bcl-xL mutant, which is defective for Bax and Bak binding but competent to bind tBid, is still cytoprotective.	bind
20446	1	6497	5	NULL	NULL	0	NULL	IgG1 mAb	NULL		bind	NULL	high affinity			GPI	NULL				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_10_3734_s_30	16505356	121 is an IgG1 mAb that binds GPI with high affinity ( Kd = 0.37 nM), and is arthritogenic when combined with other mAbs that recognize spaced epitopes on GPI ( ).	bind
24104	1	6497	7	NULL	NULL	NULL	NULL	 IgG1 mAb	GP		bind		high affinity			GPI	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_10_3734_s_30	16505356	121 is an IgG1 mAb that binds GPI with high affinity ( Kd = 0.37 nM), and is arthritogenic when combined with other mAbs that recognize spaced epitopes on GPI ( ).	bind
20451	1	6498	5	10	NULL	0	NULL	C/EBPdelta			acts as				APRE site in promoter					IL-6-inducible element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2108_s_420	9528783	121:731-738, 1997) have also identified the APRE site in the C/EBPdelta promoter as an IL-6-inducible element that binds Stat3.	bind
20452	2	6498	5	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL				Stat3	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_4_2108_s_420	9528783	121:731-738, 1997) have also identified the APRE site in the C/EBPdelta promoter as an IL-6-inducible element that binds Stat3.	bind
24107	2	6498	7	NULL	NULL	NULL	NULL	statement 1	Process		binds					Stat3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2108_s_420	9528783	121:731-738, 1997) have also identified the APRE site in the C/EBPdelta promoter as an IL-6-inducible element that binds Stat3.	bind
24108	1	6498	7	NULL	NULL	NULL	NULL	C/EBPdelta	GP		acts as				APRE site in the promoter					 IL-6-inducible element 	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_2108_s_420	9528783	121:731-738, 1997) have also identified the APRE site in the C/EBPdelta promoter as an IL-6-inducible element that binds Stat3.	bind
20453	1	6499	5	NULL	NULL	0	NULL	sHSP60	NULL	human	bind	NULL				TLR4/CD14	NULL				NULL	in human mononuclear cells	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_10_1547_s_218	12377729	122 -  127 In human mononuclear cells, human sHSP60 binds to TLR4/CD14, leading to p38 MAPK activation, 122 whereas in smooth muscle and epithelial cells, chlamydial and human sHSP60 stimulates ERK42/44 activation.	bind
20454	2	6499	5	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				p38 MAPK	NULL	activation of			NULL	in human mononuclear cells	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_10_1547_s_218	12377729	122 -  127 In human mononuclear cells, human sHSP60 binds to TLR4/CD14, leading to p38 MAPK activation, 122 whereas in smooth muscle and epithelial cells, chlamydial and human sHSP60 stimulates ERK42/44 activation.	bind
20455	3	6499	5	NULL	NULL	0	NULL	sHSP60	NULL	chlamydial	stimulates	NULL				ERK42/44	NULL	activation of			NULL	in smooth muscle	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_10_1547_s_218	12377729	122 -  127 In human mononuclear cells, human sHSP60 binds to TLR4/CD14, leading to p38 MAPK activation, 122 whereas in smooth muscle and epithelial cells, chlamydial and human sHSP60 stimulates ERK42/44 activation.	bind
20457	4	6499	5	NULL	NULL	0	NULL	sHSP60	NULL	human	stimulates	NULL				ERK42/44	NULL	activation of			NULL	in smooth muscle	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_10_1547_s_218	12377729	122 -  127 In human mononuclear cells, human sHSP60 binds to TLR4/CD14, leading to p38 MAPK activation, 122 whereas in smooth muscle and epithelial cells, chlamydial and human sHSP60 stimulates ERK42/44 activation.	bind
20458	5	6499	5	NULL	NULL	0	NULL	sHSP60	NULL	chlamydial	stimulates	NULL				ERK42/44	NULL	activation of			NULL	in epithelial cells	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_10_1547_s_218	12377729	122 -  127 In human mononuclear cells, human sHSP60 binds to TLR4/CD14, leading to p38 MAPK activation, 122 whereas in smooth muscle and epithelial cells, chlamydial and human sHSP60 stimulates ERK42/44 activation.	bind
20459	6	6499	5	NULL	NULL	0	NULL	sHSP60	NULL	human	stimulates	NULL				ERK42/44	NULL	activation of			NULL	in epithelial cells	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_10_1547_s_218	12377729	122 -  127 In human mononuclear cells, human sHSP60 binds to TLR4/CD14, leading to p38 MAPK activation, 122 whereas in smooth muscle and epithelial cells, chlamydial and human sHSP60 stimulates ERK42/44 activation.	bind
24109	1	6499	7	NULL	NULL	NULL	NULL	sHSP60	GP	human 	bind					TLR4/CD14	Cell				NULL	human mononuclear cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_10_1547_s_218	12377729	122 -  127 In human mononuclear cells, human sHSP60 binds to TLR4/CD14, leading to p38 MAPK activation, 122 whereas in smooth muscle and epithelial cells, chlamydial and human sHSP60 stimulates ERK42/44 activation.	bind
24110	2	6499	7	NULL	NULL	NULL	NULL	statement 1	Process		leads to					p38 MAPK	GP	activation of			NULL	human mononuclear cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_10_1547_s_218	12377729	122 -  127 In human mononuclear cells, human sHSP60 binds to TLR4/CD14, leading to p38 MAPK activation, 122 whereas in smooth muscle and epithelial cells, chlamydial and human sHSP60 stimulates ERK42/44 activation.	bind
24111	3	6499	7	NULL	NULL	NULL	NULL	sHSP60	GP	human	stimulates					ERK42/44	GP	activation of			NULL	smooth muscle cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_10_1547_s_218	12377729	122 -  127 In human mononuclear cells, human sHSP60 binds to TLR4/CD14, leading to p38 MAPK activation, 122 whereas in smooth muscle and epithelial cells, chlamydial and human sHSP60 stimulates ERK42/44 activation.	bind
24112	4	6499	7	NULL	NULL	NULL	NULL	sHSP60	GP	human	stimulates					ERK42/44	GP	activation of			NULL	epithelial cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_10_1547_s_218	12377729	122 -  127 In human mononuclear cells, human sHSP60 binds to TLR4/CD14, leading to p38 MAPK activation, 122 whereas in smooth muscle and epithelial cells, chlamydial and human sHSP60 stimulates ERK42/44 activation.	bind
24113	5	6499	7	NULL	NULL	NULL	NULL	sHSP60	GP	chlamydial	stimulates					ERK42/44	GP	activation of			NULL	smooth muscle cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_10_1547_s_218	12377729	122 -  127 In human mononuclear cells, human sHSP60 binds to TLR4/CD14, leading to p38 MAPK activation, 122 whereas in smooth muscle and epithelial cells, chlamydial and human sHSP60 stimulates ERK42/44 activation.	bind
24114	6	6499	7	NULL	NULL	NULL	NULL	sHSP60	GP	chlamydial	stimulates					ERK42/44	GP	activation of			NULL	epithelial cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_10_1547_s_218	12377729	122 -  127 In human mononuclear cells, human sHSP60 binds to TLR4/CD14, leading to p38 MAPK activation, 122 whereas in smooth muscle and epithelial cells, chlamydial and human sHSP60 stimulates ERK42/44 activation.	bind
20460	1	6500	5	NULL	NULL	0	NULL	PBR gene	NULL	disruption	blocks	NULL				steroidogenesis	NULL				NULL	in Leydig cells	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1150_s_289	15130918	124 Many lines of experimental evidence have implicated this protein in mitochondrial cholesterol transport: PBR gene disruption in Leydig cells blocks steroidogenesis, PBR binds cholesterol with high affinity, bacteria expressing PBR take-up cholesterol, and PBR ligands stimulate steroidogenesis and 27-hydroxycholesterol formation.	bind
20461	2	6500	5	NULL	NULL	0	NULL	PBR	NULL		bind	NULL	high affinity			cholesterol	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1150_s_289	15130918	124 Many lines of experimental evidence have implicated this protein in mitochondrial cholesterol transport: PBR gene disruption in Leydig cells blocks steroidogenesis, PBR binds cholesterol with high affinity, bacteria expressing PBR take-up cholesterol, and PBR ligands stimulate steroidogenesis and 27-hydroxycholesterol formation.	bind
20462	3	6500	5	NULL	NULL	0	NULL	bacteria	NULL	expressing PBR	take-up	NULL				cholesterol	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1150_s_289	15130918	124 Many lines of experimental evidence have implicated this protein in mitochondrial cholesterol transport: PBR gene disruption in Leydig cells blocks steroidogenesis, PBR binds cholesterol with high affinity, bacteria expressing PBR take-up cholesterol, and PBR ligands stimulate steroidogenesis and 27-hydroxycholesterol formation.	bind
20463	4	6500	5	NULL	NULL	0	NULL	PBR ligands	NULL		stimulates	NULL				steroidogenesis	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1150_s_289	15130918	124 Many lines of experimental evidence have implicated this protein in mitochondrial cholesterol transport: PBR gene disruption in Leydig cells blocks steroidogenesis, PBR binds cholesterol with high affinity, bacteria expressing PBR take-up cholesterol, and PBR ligands stimulate steroidogenesis and 27-hydroxycholesterol formation.	bind
20464	5	6500	5	NULL	NULL	0	NULL	PBR ligands	NULL		stimulates	NULL				27-hydroxycholesterol	NULL	formation of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1150_s_289	15130918	124 Many lines of experimental evidence have implicated this protein in mitochondrial cholesterol transport: PBR gene disruption in Leydig cells blocks steroidogenesis, PBR binds cholesterol with high affinity, bacteria expressing PBR take-up cholesterol, and PBR ligands stimulate steroidogenesis and 27-hydroxycholesterol formation.	bind
24115	1	6500	7	NULL	NULL	NULL	NULL	PBR gene	GP	disruption in	blocks					steroidogenesis	Process				NULL	Leydig cells	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1150_s_289	15130918	124 Many lines of experimental evidence have implicated this protein in mitochondrial cholesterol transport: PBR gene disruption in Leydig cells blocks steroidogenesis, PBR binds cholesterol with high affinity, bacteria expressing PBR take-up cholesterol, and PBR ligands stimulate steroidogenesis and 27-hydroxycholesterol formation.	bind
24116	2	6500	7	NULL	NULL	NULL	NULL	PBR	GP		binds		high affinity			cholesterol	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1150_s_289	15130918	124 Many lines of experimental evidence have implicated this protein in mitochondrial cholesterol transport: PBR gene disruption in Leydig cells blocks steroidogenesis, PBR binds cholesterol with high affinity, bacteria expressing PBR take-up cholesterol, and PBR ligands stimulate steroidogenesis and 27-hydroxycholesterol formation.	bind
24117	3	6500	7	NULL	NULL	NULL	NULL	PBR	GP	bacteria expressing 	take-up					cholesterol	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1150_s_289	15130918	124 Many lines of experimental evidence have implicated this protein in mitochondrial cholesterol transport: PBR gene disruption in Leydig cells blocks steroidogenesis, PBR binds cholesterol with high affinity, bacteria expressing PBR take-up cholesterol, and PBR ligands stimulate steroidogenesis and 27-hydroxycholesterol formation.	bind
24118	4	6500	7	NULL	NULL	NULL	NULL	PBR ligands	GP		stimulate					steroidogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1150_s_289	15130918	124 Many lines of experimental evidence have implicated this protein in mitochondrial cholesterol transport: PBR gene disruption in Leydig cells blocks steroidogenesis, PBR binds cholesterol with high affinity, bacteria expressing PBR take-up cholesterol, and PBR ligands stimulate steroidogenesis and 27-hydroxycholesterol formation.	bind
24119	5	6500	7	NULL	NULL	NULL	NULL	PBR ligands	GP		stimulate					27-hydroxycholesterol	Chemical	formation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1150_s_289	15130918	124 Many lines of experimental evidence have implicated this protein in mitochondrial cholesterol transport: PBR gene disruption in Leydig cells blocks steroidogenesis, PBR binds cholesterol with high affinity, bacteria expressing PBR take-up cholesterol, and PBR ligands stimulate steroidogenesis and 27-hydroxycholesterol formation.	bind
20465	1	6502	5	10	NULL	0	NULL	CK18		I 125 labelled	bind					trypomastigote cells		T. cruzi			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_22_19382_s_202	11278913	125 I-CK18 binds to  T. cruzi trypomastigote cells.	bind
24178	1	6502	7	NULL	NULL	NULL	NULL	CK18	GP	I 125 labelled	binds to					trypomastigote cells	Cell	T. cruzi			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_22_19382_s_202	11278913	125 I-CK18 binds to  T. cruzi trypomastigote cells.	bind
20466	1	6503	5	NULL	NULL	0	NULL	125 I-hCG	NULL		bind	NULL				LH/CG Receptor	NULL	solubilized			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_22_13835_s_45	9593728	125 I-hCG Binding to Solubilized LH/CG Receptor-- Transfected cells were washed twice with ice-cold 150 mM NaCl and 20 mM HEPES, pH 7.4 (buffer A).	bind
24179	1	6503	7	NULL	NULL	NULL	NULL	125 I-hCG	GP		bind					LH/CG Receptor	GP	solubilized			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_22_13835_s_45	9593728	125 I-hCG Binding to Solubilized LH/CG Receptor-- Transfected cells were washed twice with ice-cold 150 mM NaCl and 20 mM HEPES, pH 7.4 (buffer A).	bind
20467	1	6505	5	NULL	NULL	0	NULL	Bowes melanoma cells	NULL		is transfected with	NULL				LIMPII cDNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_4855_s_146	9478926	125 I-TSP1 binds to Bowes melanoma cells transfected with LIMPII cDNA.	bind
20468	2	6505	5	NULL	NULL	0	NULL	125 I-TSP1	NULL		bind	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_4855_s_146	9478926	125 I-TSP1 binds to Bowes melanoma cells transfected with LIMPII cDNA.	bind
24180	1	6505	7	NULL	NULL	NULL	NULL	Bowes melanoma cells	Cell		transfected with					LIMPII cDNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_9_4855_s_146	9478926	125 I-TSP1 binds to Bowes melanoma cells transfected with LIMPII cDNA.	bind
24181	2	6505	7	NULL	NULL	NULL	NULL	125 I-TSP1	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_9_4855_s_146	9478926	125 I-TSP1 binds to Bowes melanoma cells transfected with LIMPII cDNA.	bind
20469	1	6506	5	NULL	NULL	0	NULL	125 I-VEGF145	NULL		bind	NULL				np-2 receptors	NULL				NULL	on endothelial cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_24_18040_s_152	10748121	125 I-VEGF145 binding differentiates between  np-2  and  np-1  receptors on endothelial cells and breast cancer cells.	bind
20470	2	6506	5	NULL	NULL	0	NULL	125 I-VEGF145	NULL		bind	NULL				np-1 receptors	NULL				NULL	on endothelial cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_24_18040_s_152	10748121	125 I-VEGF145 binding differentiates between  np-2  and  np-1  receptors on endothelial cells and breast cancer cells.	bind
20471	3	6506	5	NULL	NULL	0	NULL	125 I-VEGF145	NULL		bind	NULL				np-2 receptors	NULL				NULL	on breast cancer cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_24_18040_s_152	10748121	125 I-VEGF145 binding differentiates between  np-2  and  np-1  receptors on endothelial cells and breast cancer cells.	bind
20472	4	6506	5	NULL	NULL	0	NULL	125 I-VEGF145	NULL		bind	NULL				np-1 receptors	NULL				NULL	on breast cancer cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_24_18040_s_152	10748121	125 I-VEGF145 binding differentiates between  np-2  and  np-1  receptors on endothelial cells and breast cancer cells.	bind
24182	1	6506	7	NULL	NULL	NULL	NULL	125 I-VEGF145	GP		bind					np-2 receptor	GP				NULL	endothelial cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_24_18040_s_152	10748121	125 I-VEGF145 binding differentiates between  np-2  and  np-1  receptors on endothelial cells and breast cancer cells.	bind
24183	2	6506	7	NULL	NULL	NULL	NULL	125 I-VEGF145	GP		bind					np-1 receptor	GP				NULL	endothelial cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_24_18040_s_152	10748121	125 I-VEGF145 binding differentiates between  np-2  and  np-1  receptors on endothelial cells and breast cancer cells.	bind
24184	3	6506	7	NULL	NULL	NULL	NULL	125 I-VEGF145	GP		bind					np-2 receptor	GP				NULL	breast cancer cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_24_18040_s_152	10748121	125 I-VEGF145 binding differentiates between  np-2  and  np-1  receptors on endothelial cells and breast cancer cells.	bind
24185	4	6506	7	NULL	NULL	NULL	NULL	125 I-VEGF145	GP		bind					np-1 receptor	GP				NULL	breast cancer cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_24_18040_s_152	10748121	125 I-VEGF145 binding differentiates between  np-2  and  np-1  receptors on endothelial cells and breast cancer cells.	bind
20476	1	6507	5	NULL	NULL	0	NULL	Hb	NULL		bind	NULL				BCE surface proteins	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_8_2528_s_172	12670977	125/CE and 65/CE, positive controls where IgG 125 and 65 were used  to neutralize Hb binding of the BCE surface proteins; 125/HA2 and 65/HA2, same assay  after rHA2-bound resin had been used to deplete rHA2-related IgG from IgG 125 and  65, resulting in a shift in the profile of the curves.	bind
30267	2	6507	5	NULL	NULL	0	NULL	IgG 125	NULL		neutralize	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_8_2528_s_172	12670977	125/CE and 65/CE, positive controls where IgG 125 and 65 were used  to neutralize Hb binding of the BCE surface proteins; 125/HA2 and 65/HA2, same assay  after rHA2-bound resin had been used to deplete rHA2-related IgG from IgG 125 and  65, resulting in a shift in the profile of the curves.	bind
30268	3	6507	5	NULL	NULL	0	NULL	IgG 65	NULL		neutralize	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_8_2528_s_172	12670977	125/CE and 65/CE, positive controls where IgG 125 and 65 were used  to neutralize Hb binding of the BCE surface proteins; 125/HA2 and 65/HA2, same assay  after rHA2-bound resin had been used to deplete rHA2-related IgG from IgG 125 and  65, resulting in a shift in the profile of the curves.	bind
24186	1	6507	7	NULL	NULL	NULL	NULL	Hb	GP		bind					BCE surface protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_8_2528_s_172	12670977	125/CE and 65/CE, positive controls where IgG 125 and 65 were used  to neutralize Hb binding of the BCE surface proteins; 125/HA2 and 65/HA2, same assay  after rHA2-bound resin had been used to deplete rHA2-related IgG from IgG 125 and  65, resulting in a shift in the profile of the curves.	bind
24187	2	6507	7	NULL	NULL	NULL	NULL	IgG 125	GP		neutralize					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_8_2528_s_172	12670977	125/CE and 65/CE, positive controls where IgG 125 and 65 were used  to neutralize Hb binding of the BCE surface proteins; 125/HA2 and 65/HA2, same assay  after rHA2-bound resin had been used to deplete rHA2-related IgG from IgG 125 and  65, resulting in a shift in the profile of the curves.	bind
24188	3	6507	7	NULL	NULL	NULL	NULL	IgG 65	GP		neutralize					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_8_2528_s_172	12670977	125/CE and 65/CE, positive controls where IgG 125 and 65 were used  to neutralize Hb binding of the BCE surface proteins; 125/HA2 and 65/HA2, same assay  after rHA2-bound resin had been used to deplete rHA2-related IgG from IgG 125 and  65, resulting in a shift in the profile of the curves.	bind
20479	1	6509	5	NULL	NULL	0	NULL	pili	NULL	125I labeled	bind	NULL				CEPs	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_invest-ophthalmol-vis-sci_36_3_7890494_s_13	7890494	125I labeling of pili and a solid-phase  binding assay confirmed that pili bind to CEPs and, further, that binding  could be competitively inhibited by excess unlabeled pili and that the  receptors appeared saturable.	bind
20482	2	6509	5	NULL	NULL	0	NULL	pili	NULL	unlabeled	bind	NULL				CEPs	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_invest-ophthalmol-vis-sci_36_3_7890494_s_13	7890494	125I labeling of pili and a solid-phase  binding assay confirmed that pili bind to CEPs and, further, that binding  could be competitively inhibited by excess unlabeled pili and that the  receptors appeared saturable.	bind
20484	3	6509	5	NULL	NULL	0	NULL	statement 2	NULL		inhibits	NULL	competitively			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_invest-ophthalmol-vis-sci_36_3_7890494_s_13	7890494	125I labeling of pili and a solid-phase  binding assay confirmed that pili bind to CEPs and, further, that binding  could be competitively inhibited by excess unlabeled pili and that the  receptors appeared saturable.	bind
24189	1	6509	7	NULL	NULL	NULL	NULL	pili	OrganismPart	125I labeled	bind					CEPs	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_invest-ophthalmol-vis-sci_36_3_7890494_s_13	7890494	125I labeling of pili and a solid-phase  binding assay confirmed that pili bind to CEPs and, further, that binding  could be competitively inhibited by excess unlabeled pili and that the  receptors appeared saturable.	bind
24190	2	6509	7	NULL	NULL	NULL	NULL	pili	OrganismPart	unlabeled	bind					CEPs	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_invest-ophthalmol-vis-sci_36_3_7890494_s_13	7890494	125I labeling of pili and a solid-phase  binding assay confirmed that pili bind to CEPs and, further, that binding  could be competitively inhibited by excess unlabeled pili and that the  receptors appeared saturable.	bind
24191	3	6509	7	NULL	NULL	NULL	NULL	statement 2	Process		inhibits		competitively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_invest-ophthalmol-vis-sci_36_3_7890494_s_13	7890494	125I labeling of pili and a solid-phase  binding assay confirmed that pili bind to CEPs and, further, that binding  could be competitively inhibited by excess unlabeled pili and that the  receptors appeared saturable.	bind
20485	1	6510	5	NULL	NULL	0	NULL	125I- -Conotoxin	NULL		bind	NULL	specifically			cells	NULL				NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_188_1_97_s_76	10867241	125I- -Conotoxin specifically bound to Tris-EDTA-permeabilized cells with saturation kinetics.	bind
24192	1	6510	7	NULL	NULL	NULL	NULL	125I- -Conotoxin	Chemical		bind		specifically			cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_188_1_97_s_76	10867241	125I- -Conotoxin specifically bound to Tris-EDTA-permeabilized cells with saturation kinetics.	bind
20486	1	6511	5	NULL	NULL	0	NULL	125I-Abeta	NULL		is cross-linked to	NULL	covalently			alpha2M-MA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_13338_s_101	11823454	125I-Abeta that was covalently cross-linked to alpha2M-MA (bound) and free 125I-Abeta (free), which includes free Abeta and Abeta that was bound to alpha2M-MA but not cross-linked, were quantitated by PhosphorImager analysis.	bind
24193	1	6511	7	NULL	NULL	NULL	NULL	125I-Abeta	GP		bind					alpha2M-MA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_13338_s_101	11823454	125I-Abeta that was covalently cross-linked to alpha2M-MA (bound) and free 125I-Abeta (free), which includes free Abeta and Abeta that was bound to alpha2M-MA but not cross-linked, were quantitated by PhosphorImager analysis.	bind
20489	1	6512	5	NULL	NULL	0	NULL	TIMP-2	NULL		bind	NULL				MMP 	NULL		active sites		NULL		NULL	NULL	NULL	NULL	gw60_cell_114_2_171_s_101	12887919	125I-Ala+TIMP-2 was utilized in these experiments to reduce potential background from TIMP-2 binding to MMP active sites  (Hoegy et al., 2001  ).	bind
24194	1	6512	7	NULL	NULL	NULL	NULL	 TIMP-2	GP		bind					MMP	GP		active site		NULL		NULL	NULL	NULL	NULL	gw60_cell_114_2_171_s_101	12887919	125I-Ala+TIMP-2 was utilized in these experiments to reduce potential background from TIMP-2 binding to MMP active sites  (Hoegy et al., 2001  ).	bind
20490	1	6513	5	NULL	NULL	0	NULL	125I-alpha-BGT	NULL		bind	NULL				neonatal muscle cells	NULL				NULL	in culture	NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_281_3_1463_s_63	9190884	125I-alpha-BGT binding to neonatal muscle cells in culture.	bind
24195	1	6513	7	NULL	NULL	NULL	NULL	125I-alpha-BGT	GP		binds to					neonatal muscle cells	Cell				NULL	in culture	NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_281_3_1463_s_63	9190884	125I-alpha-BGT binding to neonatal muscle cells in culture.	bind
20491	1	6514	5	NULL	NULL	0	NULL	125I-aminopeptidase	NULL		bind	NULL				Cry1Ab	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_5_2106_s_8	11976078	125I-aminopeptidase bound Cry1Ab to a limited extent but not the Cry1Ab domain I mutant Y153D or Cry1Ca.	bind
20492	2	6514	5	NULL	NULL	0	NULL	Cry1Ab	NULL	mutant	does not bind	NULL		domain I Y153D		125I-aminopeptidase	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_5_2106_s_8	11976078	125I-aminopeptidase bound Cry1Ab to a limited extent but not the Cry1Ab domain I mutant Y153D or Cry1Ca.	bind
20493	3	6514	5	NULL	NULL	0	NULL	Cry1Ca	NULL		does not bind	NULL				125I-aminopeptidase	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_5_2106_s_8	11976078	125I-aminopeptidase bound Cry1Ab to a limited extent but not the Cry1Ab domain I mutant Y153D or Cry1Ca.	bind
24196	1	6514	7	NULL	NULL	NULL	NULL	125I-aminopeptidase	GP		bind					Cry1Ab	GP				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_68_5_2106_s_8	11976078	125I-aminopeptidase bound Cry1Ab to a limited extent but not the Cry1Ab domain I mutant Y153D or Cry1Ca.	bind
24197	2	6514	7	NULL	NULL	NULL	NULL	125I-aminopeptidase	GP		does not bind					Cry1Ab	GP	mutant 	domain I Y153D		NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_68_5_2106_s_8	11976078	125I-aminopeptidase bound Cry1Ab to a limited extent but not the Cry1Ab domain I mutant Y153D or Cry1Ca.	bind
24198	3	6514	7	NULL	NULL	NULL	NULL	125I-aminopeptidase	GP		does not bind					Cry1Ca	GP				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_68_5_2106_s_8	11976078	125I-aminopeptidase bound Cry1Ab to a limited extent but not the Cry1Ab domain I mutant Y153D or Cry1Ca.	bind
24722	1	6515	5	NULL	NULL	0	NULL	125I-Ang IV	NULL		bind	NULL				MDBK	NULL	cell membranes of			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
24723	2	6515	5	NULL	NULL	0	NULL	losartan	NULL		is antagonist of	NULL				AT1 receptor	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
24724	3	6515	5	NULL	NULL	0	NULL	statement 1	NULL		is unaffected by	NULL				losartan	NULL				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
24725	4	6515	5	NULL	NULL	0	NULL	PD 123177	NULL		is antagonist of	NULL				AT2 receptor	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
24726	5	6515	5	NULL	NULL	0	NULL	statement 1	NULL		is unaffected by	NULL				PD 123177	NULL				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
24727	6	6515	5	NULL	NULL	0	NULL	Sar1,Thr8 Ang II	NULL		is antagonist of	NULL				AT1/AT2 receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
24728	7	6515	5	NULL	NULL	0	NULL	statement 1	NULL		is unaffected by	NULL				Sar1,Thr8 Ang II	NULL				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
24729	8	6515	5	NULL	NULL	0	NULL	Sar1,Ile8 Ang II	NULL		is antagonist of	NULL				AT1/AT2 receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
24730	9	6515	5	NULL	NULL	0	NULL	statement 1	NULL		is unaffected by	NULL				Sar1,Ile8 Ang II	NULL				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
24731	10	6515	5	NULL	NULL	0	NULL	D-Ala7 Ang(1-7)	NULL		is antagonist of	NULL	putative			Ang(1-7) receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
24732	11	6515	5	NULL	NULL	0	NULL	statement 1	NULL		is unaffected by	NULL				D-Ala7 Ang(1-7)	NULL				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
24733	12	6515	5	NULL	NULL	0	NULL	divalinal Ang IV 	NULL		is antagonist of	NULL	putative			AT4 receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
24734	13	6515	5	NULL	NULL	0	NULL	divalinal Ang IV 	NULL		bind	NULL					NULL		125I-Ang IV binding site		NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
24735	14	6515	5	NULL	NULL	0	NULL	NleYI-6-hexamide	NULL		is antagonist of	NULL	putative			AT4 receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
24736	15	6515	5	NULL	NULL	0	NULL	NleYI-6-hexamide	NULL		bind	NULL					NULL		125I-Ang IV binding site		NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
24737	16	6515	5	NULL	NULL	0	NULL	statement 13	NULL		competes with	NULL	high affinity			statement 15	NULL				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
24199	1	6515	7	NULL	NULL	NULL	NULL	125I-Ang IV	GP		bind					MDBK	GP	cell membrane of			NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
24200	3	6515	7	NULL	NULL	NULL	NULL	statement 1	Process		is unaffected by					losartan 	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
24201	5	6515	7	NULL	NULL	NULL	NULL	statement 1	Process		is unaffected by					PD 123177	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
24203	7	6515	7	NULL	NULL	NULL	NULL	statement 1	Process		is unaffected by					Sar1,Thr8 Ang II	GP				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
24204	8	6515	7	NULL	NULL	NULL	NULL	Sar1,Ile8 Ang II 	GP		is antagonist of					AT1/AT2 receptor 	GP				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
31336	2	6515	7	NULL	NULL	NULL	NULL	losartan 	Chemical		is  antagonist of					AT1 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
31337	4	6515	7	NULL	NULL	NULL	NULL	PD 123177	Chemical		is antagonist of					AT2 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
31338	6	6515	7	NULL	NULL	NULL	NULL	Sar1,Thr8 Ang II	GP		is antagonist of					AT1/AT2 receptor 	GP				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
31339	10	6515	7	NULL	NULL	NULL	NULL	D-Ala7 Ang(1-7)	GP		is antagonist of					putative Ang(1-7) receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
31340	12	6515	7	NULL	NULL	NULL	NULL	divalinal Ang IV	GP		is antagonist of					putative AT4 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
31341	13	6515	7	NULL	NULL	NULL	NULL	NleYI-6-hexamide	Chemical		is antagonist of					putative AT4 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
31342	9	6515	7	NULL	NULL	NULL	NULL	statement 1	Process		is unaffected by					Sar1,Ile8 Ang II 	GP				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
31343	11	6515	7	NULL	NULL	NULL	NULL	statement 1	Process		is unaffected by					D-Ala7 Ang(1-7) 	GP				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
31344	14	6515	7	NULL	NULL	NULL	NULL	divalinal Ang IV	GP		bind		high affinity			125I-Ang IV	GP				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
31345	15	6515	7	NULL	NULL	NULL	NULL	NleYI-6-hexamide	Chemical		bind		high affinity			125I-Ang IV 	GP				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
31346	16	6515	7	NULL	NULL	NULL	NULL	statement 14	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
31347	17	6515	7	NULL	NULL	NULL	NULL	statement 15	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_1242_s_104	10565848	125I-Ang IV binding to MDBK cell membranes was largely unaffected by losartan (AT1 receptor antagonist), PD 123177 (AT2 receptor antagonist), Sar1,Thr8 Ang II and Sar1,Ile8 Ang II (both AT1/AT2 receptor antagonists), or D-Ala7 Ang(1-7) [putative Ang(1-7) receptor antagonist], whereas divalinal Ang IV and NleYI-6-hexamide (both putative AT4 receptor antagonists) competed with high affinity for the 125I-Ang IV binding site.	bind
20495	1	6516	5	NULL	NULL	0	NULL	125I-Anti-CK18 IgG	NULL		bind	NULL				HTC cells	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_45_28574_s_162	9353322	125I-Anti-CK18 IgG bound to HTC cells to a much greater extent than preimmune IgG, and comparable results were obtained with HepG2 cells.	bind
20496	2	6516	5	NULL	NULL	0	NULL	preimmune IgG	NULL		bind	NULL				HTC cells	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_45_28574_s_162	9353322	125I-Anti-CK18 IgG bound to HTC cells to a much greater extent than preimmune IgG, and comparable results were obtained with HepG2 cells.	bind
20497	3	6516	5	NULL	NULL	0	NULL	statement 1	NULL		greater than	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_45_28574_s_162	9353322	125I-Anti-CK18 IgG bound to HTC cells to a much greater extent than preimmune IgG, and comparable results were obtained with HepG2 cells.	bind
20498	4	6516	5	NULL	NULL	0	NULL	125I-Anti-CK18 IgG	NULL		bind	NULL				HepG2 cells	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_45_28574_s_162	9353322	125I-Anti-CK18 IgG bound to HTC cells to a much greater extent than preimmune IgG, and comparable results were obtained with HepG2 cells.	bind
20499	5	6516	5	NULL	NULL	0	NULL	preimmune IgG	NULL		bind	NULL				HepG2 cells	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_45_28574_s_162	9353322	125I-Anti-CK18 IgG bound to HTC cells to a much greater extent than preimmune IgG, and comparable results were obtained with HepG2 cells.	bind
20500	6	6516	5	NULL	NULL	0	NULL	statement 1	NULL		is comparable to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_45_28574_s_162	9353322	125I-Anti-CK18 IgG bound to HTC cells to a much greater extent than preimmune IgG, and comparable results were obtained with HepG2 cells.	bind
20501	7	6516	5	NULL	NULL	0	NULL	statement 2	NULL		is comparable to	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_45_28574_s_162	9353322	125I-Anti-CK18 IgG bound to HTC cells to a much greater extent than preimmune IgG, and comparable results were obtained with HepG2 cells.	bind
24207	1	6516	7	NULL	NULL	NULL	NULL	125I-Anti-CK18 IgG	GP		bind					 HTC cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_45_28574_s_162	9353322	125I-Anti-CK18 IgG bound to HTC cells to a much greater extent than preimmune IgG, and comparable results were obtained with HepG2 cells.	bind
24208	2	6516	7	NULL	NULL	NULL	NULL	preimmune IgG	GP		bind					HTC cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_45_28574_s_162	9353322	125I-Anti-CK18 IgG bound to HTC cells to a much greater extent than preimmune IgG, and comparable results were obtained with HepG2 cells.	bind
24209	3	6516	7	NULL	NULL	NULL	NULL	statement 1	Process		is greater than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_45_28574_s_162	9353322	125I-Anti-CK18 IgG bound to HTC cells to a much greater extent than preimmune IgG, and comparable results were obtained with HepG2 cells.	bind
24210	4	6516	7	NULL	NULL	NULL	NULL	125I-Anti-CK18 IgG	GP		bind					HepG2 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_45_28574_s_162	9353322	125I-Anti-CK18 IgG bound to HTC cells to a much greater extent than preimmune IgG, and comparable results were obtained with HepG2 cells.	bind
31348	5	6516	7	NULL	NULL	NULL	NULL	preimmune IgG	GP		bind					HepG2 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_45_28574_s_162	9353322	125I-Anti-CK18 IgG bound to HTC cells to a much greater extent than preimmune IgG, and comparable results were obtained with HepG2 cells.	bind
20502	1	6517	5	NULL	NULL	0	NULL	125I-b-FGF	NULL		bind	NULL				V3wt-Rg	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_4_2511_s_197	9891022	125I-b-FGF Binds V3wt-Rg but Not V3mut-Rg-- Previously we demonstrated that b-FGF can bind HS-modified CD44 produced in COS cells ( 4).	bind
20503	2	6517	5	NULL	NULL	0	NULL	125I-b-FGF	NULL		does not bind	NULL				V3mut-Rg	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_4_2511_s_197	9891022	125I-b-FGF Binds V3wt-Rg but Not V3mut-Rg-- Previously we demonstrated that b-FGF can bind HS-modified CD44 produced in COS cells ( 4).	bind
20504	3	6517	5	10	NULL	0	NULL	b-FGF	NULL		bind	NULL				CD44	NULL	HS-modified			NULL	COS cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_4_2511_s_197	9891022	125I-b-FGF Binds V3wt-Rg but Not V3mut-Rg-- Previously we demonstrated that b-FGF can bind HS-modified CD44 produced in COS cells ( 4).	bind
24217	1	6517	7	NULL	NULL	NULL	NULL	125I-b-FGF	GP		binds					V3-Rg 	GP	wt			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_4_2511_s_197	9891022	125I-b-FGF Binds V3wt-Rg but Not V3mut-Rg-- Previously we demonstrated that b-FGF can bind HS-modified CD44 produced in COS cells ( 4).	bind
24218	2	6517	7	NULL	NULL	NULL	NULL	125I-b-FGF	GP		does not bind					V3-Rg 	GP	mut			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_4_2511_s_197	9891022	125I-b-FGF Binds V3wt-Rg but Not V3mut-Rg-- Previously we demonstrated that b-FGF can bind HS-modified CD44 produced in COS cells ( 4).	bind
24219	3	6517	7	NULL	NULL	NULL	NULL	b-FGF	GP		bind					CD44	Cell	HS-modified			NULL	COS cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_4_2511_s_197	9891022	125I-b-FGF Binds V3wt-Rg but Not V3mut-Rg-- Previously we demonstrated that b-FGF can bind HS-modified CD44 produced in COS cells ( 4).	bind
20505	1	6518	5	NULL	NULL	0	NULL	125I-b-FGF	NULL		does not bind	NULL				V3mut-Rg	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_4_2511_s_201	9891022	125I-b-FGF did not bind to V3mut-Rg, confirming the requirement of HS for the interaction.	bind
24738	2	6518	5	NULL	NULL	0	NULL	HS	NULL		is required for	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_4_2511_s_201	9891022	125I-b-FGF did not bind to V3mut-Rg, confirming the requirement of HS for the interaction.	bind
24739	3	6518	5	NULL	NULL	0	NULL	statement 1	NULL		confirms	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_4_2511_s_201	9891022	125I-b-FGF did not bind to V3mut-Rg, confirming the requirement of HS for the interaction.	bind
24220	1	6518	7	NULL	NULL	NULL	NULL	125I-b-FGF	GP		does not bind					V3mut-Rg	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_4_2511_s_201	9891022	125I-b-FGF did not bind to V3mut-Rg, confirming the requirement of HS for the interaction.	bind
24221	2	6518	7	NULL	NULL	NULL	NULL	HS	Chemical		is required for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_4_2511_s_201	9891022	125I-b-FGF did not bind to V3mut-Rg, confirming the requirement of HS for the interaction.	bind
45754	3	6518	7	NULL	NULL	NULL	NULL	statement 1	Process		confirms					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_4_2511_s_201	9891022	125I-b-FGF did not bind to V3mut-Rg, confirming the requirement of HS for the interaction.	bind
20510	1	6519	5	NULL	NULL	0	NULL	Botrocetin	NULL		bind	NULL				VWF	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_15_11044_s_51	10753907	125I-Botrocetin Binding Assays-- Botrocetin binding to VWF was assayed according to methods of Fujimura  et al. ( 15) as described previously ( 9).	bind
24222	1	6519	7	NULL	NULL	NULL	NULL	125I-Botrocetin	Chemical		bind					VWF	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_15_11044_s_51	10753907	125I-Botrocetin Binding Assays-- Botrocetin binding to VWF was assayed according to methods of Fujimura  et al. ( 15) as described previously ( 9).	bind
20511	1	6520	5	10	NULL	0	NULL	pancreatic membranes	NULL	wild-type;; mouse	bind	NULL				CCK-8	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_103_3_383_s_169	9927499	125I-CCK-8 competition-binding experiments (Fig.  1 c) revealed that wild-type mouse pancreatic membranes bound CCK-8 with affinity in the nanomolar range: dissociation constant,  Kd = 0.18  plus-or-minus  0.03 nM (mean  plus-or-minus  SEM,  n = 3).	bind
24223	1	6520	7	NULL	NULL	NULL	NULL	pancreatic membranes	OrganismPart	wild-type;; mouse	bind					125I-CCK-8	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_103_3_383_s_169	9927499	125I-CCK-8 competition-binding experiments (Fig.  1 c) revealed that wild-type mouse pancreatic membranes bound CCK-8 with affinity in the nanomolar range: dissociation constant,  Kd = 0.18  plus-or-minus  0.03 nM (mean  plus-or-minus  SEM,  n = 3).	bind
20512	1	6522	5	NULL	NULL	0	NULL	125I-EGF	NULL		bind	NULL				ECD	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_12_10108_s_71	11796728	125I-EGF Binding to the ECD-- The binding constants of the ECD for EGF in the presence or absence of gangliosides were determined using the scintillation proximity assay (SPA) developed by Amersham Biosciences, Inc.	bind
24224	1	6522	7	NULL	NULL	NULL	NULL	125I-EGF	GP		bind								ECD		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10108_s_71	11796728	125I-EGF Binding to the ECD-- The binding constants of the ECD for EGF in the presence or absence of gangliosides were determined using the scintillation proximity assay (SPA) developed by Amersham Biosciences, Inc.	bind
20513	1	6523	5	10	NULL	0	NULL	125I-F-heparin	NULL		bind	NULL	specifically			ATIII	NULL	recombinant;; native			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_34_20935_s_141	8702852	125I-F-heparin bound to recombinant native ATIII specifically and saturably, as demonstrated by the effective competition for binding by unlabeled F-heparin.	bind
20514	2	6523	5	10	NULL	0	NULL	125I-F-heparin	NULL		bind	NULL	saturably			ATIII	NULL	recombinant;; native			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_34_20935_s_141	8702852	125I-F-heparin bound to recombinant native ATIII specifically and saturably, as demonstrated by the effective competition for binding by unlabeled F-heparin.	bind
20515	3	6523	5	10	NULL	0	NULL	F-heparin	NULL	unlabeled	bind	NULL				ATIII	NULL	recombinant;; native			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_34_20935_s_141	8702852	125I-F-heparin bound to recombinant native ATIII specifically and saturably, as demonstrated by the effective competition for binding by unlabeled F-heparin.	bind
20516	4	6523	5	NULL	NULL	0	NULL	statement 3	NULL		competes with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_34_20935_s_141	8702852	125I-F-heparin bound to recombinant native ATIII specifically and saturably, as demonstrated by the effective competition for binding by unlabeled F-heparin.	bind
24225	1	6523	7	NULL	NULL	NULL	NULL	125I-F-heparin	GP		bind		specifically			ATIII	GP	recombinant;; native			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_34_20935_s_141	8702852	125I-F-heparin bound to recombinant native ATIII specifically and saturably, as demonstrated by the effective competition for binding by unlabeled F-heparin.	bind
24226	2	6523	7	NULL	NULL	NULL	NULL	F-heparin	GP	unlabeled	bind					ATIII 	GP	recombinant;; native			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_34_20935_s_141	8702852	125I-F-heparin bound to recombinant native ATIII specifically and saturably, as demonstrated by the effective competition for binding by unlabeled F-heparin.	bind
24227	3	6523	7	NULL	NULL	NULL	NULL	125I-F-heparin 	GP		bind		saturably			ATIII	GP	recombinant;; native			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_34_20935_s_141	8702852	125I-F-heparin bound to recombinant native ATIII specifically and saturably, as demonstrated by the effective competition for binding by unlabeled F-heparin.	bind
24228	4	6523	7	NULL	NULL	NULL	NULL	statement 2	Process		compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_34_20935_s_141	8702852	125I-F-heparin bound to recombinant native ATIII specifically and saturably, as demonstrated by the effective competition for binding by unlabeled F-heparin.	bind
24229	5	6523	7	NULL	NULL	NULL	NULL	statement 2	Process		compete with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_34_20935_s_141	8702852	125I-F-heparin bound to recombinant native ATIII specifically and saturably, as demonstrated by the effective competition for binding by unlabeled F-heparin.	bind
20517	1	6524	5	NULL	NULL	0	NULL	125I-factor Xa	NULL		bind	NULL				SMC monolayers	NULL	human			NULL		0	NULL	NULL	NULL	gw60_jclininvest_101_5_993_s_127	9486969	125I-factor Xa binding to human SMC monolayers.	bind
24230	1	6524	7	NULL	NULL	NULL	NULL	125I-factor Xa	GP		bind					SMC monolayers	OrganismPart	human			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_101_5_993_s_127	9486969	125I-factor Xa binding to human SMC monolayers.	bind
20518	1	6525	5	NULL	NULL	0	NULL	125I-HI-8	NULL		does not bind	NULL				UTI-BPs	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_17_13650_s_134	11278581	125I-HI-8 failed to bind any of the UTI-BPs (data not shown), demonstrating that there was no indication that the C-domain of UTI was involved in binding of UTI to these UTI-BPs.	bind
20519	2	6525	5	NULL	NULL	0	NULL	UTI	NULL		bind	NULL				UTI-BPs	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_17_13650_s_134	11278581	125I-HI-8 failed to bind any of the UTI-BPs (data not shown), demonstrating that there was no indication that the C-domain of UTI was involved in binding of UTI to these UTI-BPs.	bind
30269	3	6525	5	NULL	NULL	0	NULL	UTI	NULL		is not involved in	NULL		C domain		statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_17_13650_s_134	11278581	125I-HI-8 failed to bind any of the UTI-BPs (data not shown), demonstrating that there was no indication that the C-domain of UTI was involved in binding of UTI to these UTI-BPs.	bind
24231	1	6525	7	NULL	NULL	NULL	NULL	125I-HI-8	GP		does not bind					UTI-BPs	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_17_13650_s_134	11278581	125I-HI-8 failed to bind any of the UTI-BPs (data not shown), demonstrating that there was no indication that the C-domain of UTI was involved in binding of UTI to these UTI-BPs.	bind
24232	2	6525	7	NULL	NULL	NULL	NULL	UTI	GP		bind					UTI-BPs	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_17_13650_s_134	11278581	125I-HI-8 failed to bind any of the UTI-BPs (data not shown), demonstrating that there was no indication that the C-domain of UTI was involved in binding of UTI to these UTI-BPs.	bind
24233	3	6525	7	NULL	NULL	NULL	NULL	 UTI	GP		is not involved in			C-domain		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_17_13650_s_134	11278581	125I-HI-8 failed to bind any of the UTI-BPs (data not shown), demonstrating that there was no indication that the C-domain of UTI was involved in binding of UTI to these UTI-BPs.	bind
20520	1	6526	5	NULL	NULL	0	NULL	125I-Hst 5	NULL		bind	NULL	saturably			SSA1/SSA2 strain	NULL	wild-type			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_31_28553_s_8	12761219	125I-Hst 5 binding assays showed saturable binding  ( K d = 2.57 x  10 - 6M) with the wild-type   SSA1/SSA2 strain; however, Hst 5 binding with the  delta ssa1ssa2 double mutant was reduced  ( K d = 1.25 x 10 - 6M).	bind
20521	2	6526	5	NULL	NULL	0	NULL	Hst 5	NULL		bind	NULL	reduced			delta ssa1ssa2	NULL	double mutant			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_31_28553_s_8	12761219	125I-Hst 5 binding assays showed saturable binding  ( K d = 2.57 x  10 - 6M) with the wild-type   SSA1/SSA2 strain; however, Hst 5 binding with the  delta ssa1ssa2 double mutant was reduced  ( K d = 1.25 x 10 - 6M).	bind
24398	1	6526	7	NULL	NULL	NULL	NULL	125I-Hst 5	GP		bind		saturably			SSA1/SSA2 strain	Organism	wild-type			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_31_28553_s_8	12761219	125I-Hst 5 binding assays showed saturable binding  ( K d = 2.57 x  10 - 6M) with the wild-type   SSA1/SSA2 strain; however, Hst 5 binding with the  delta ssa1ssa2 double mutant was reduced  ( K d = 1.25 x 10 - 6M).	bind
24399	2	6526	7	NULL	NULL	NULL	NULL	Hst 5	GP		bind		reduced			delta ssa1ssa2	Organism	double mutant			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_31_28553_s_8	12761219	125I-Hst 5 binding assays showed saturable binding  ( K d = 2.57 x  10 - 6M) with the wild-type   SSA1/SSA2 strain; however, Hst 5 binding with the  delta ssa1ssa2 double mutant was reduced  ( K d = 1.25 x 10 - 6M).	bind
20523	1	6527	5	NULL	NULL	0	NULL	anti-band 3 IgG	NULL	125I-labeled human	bind	NULL	specifically			band 3 glycoprotein	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biochem-(tokyo)_119_4_8743563_s_3	8743563	125I-labeled  human anti-band 3 IgG specifically bound to band 3 glycoprotein and lactoferrin,  a glycoprotein that has poly-N-acetyllactosamine-type sugar chains like  band 3, on the polyvinylidene difluoride blotting membrane.	bind
20524	2	6527	5	NULL	NULL	0	NULL	anti-band 3 IgG	NULL	125I-labeled human	bind	NULL	specifically			lactoferrin	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biochem-(tokyo)_119_4_8743563_s_3	8743563	125I-labeled  human anti-band 3 IgG specifically bound to band 3 glycoprotein and lactoferrin,  a glycoprotein that has poly-N-acetyllactosamine-type sugar chains like  band 3, on the polyvinylidene difluoride blotting membrane.	bind
20525	3	6527	5	NULL	NULL	0	NULL	lactoferrin	NULL		contains	NULL				poly-N-acetyllactosamine-type sugar chains	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biochem-(tokyo)_119_4_8743563_s_3	8743563	125I-labeled  human anti-band 3 IgG specifically bound to band 3 glycoprotein and lactoferrin,  a glycoprotein that has poly-N-acetyllactosamine-type sugar chains like  band 3, on the polyvinylidene difluoride blotting membrane.	bind
30270	4	6527	5	NULL	NULL	0	NULL	lactoferrin	NULL		is a type of	NULL				glycoprotein	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biochem-(tokyo)_119_4_8743563_s_3	8743563	125I-labeled  human anti-band 3 IgG specifically bound to band 3 glycoprotein and lactoferrin,  a glycoprotein that has poly-N-acetyllactosamine-type sugar chains like  band 3, on the polyvinylidene difluoride blotting membrane.	bind
24400	1	6527	7	NULL	NULL	NULL	NULL	anti-band 3 IgG	GP	125I-labeled human	bind		specifically			band 3 glycoprotein	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biochem-(tokyo)_119_4_8743563_s_3	8743563	125I-labeled  human anti-band 3 IgG specifically bound to band 3 glycoprotein and lactoferrin,  a glycoprotein that has poly-N-acetyllactosamine-type sugar chains like  band 3, on the polyvinylidene difluoride blotting membrane.	bind
24401	2	6527	7	NULL	NULL	NULL	NULL	anti-band 3 IgG	GP	125I-labeled human	bind		specifically			lactoferrin	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biochem-(tokyo)_119_4_8743563_s_3	8743563	125I-labeled  human anti-band 3 IgG specifically bound to band 3 glycoprotein and lactoferrin,  a glycoprotein that has poly-N-acetyllactosamine-type sugar chains like  band 3, on the polyvinylidene difluoride blotting membrane.	bind
24402	3	6527	7	NULL	NULL	NULL	NULL	lactoferrin	GP		contains					poly-N-acetyllactosamine-type sugar chains	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biochem-(tokyo)_119_4_8743563_s_3	8743563	125I-labeled  human anti-band 3 IgG specifically bound to band 3 glycoprotein and lactoferrin,  a glycoprotein that has poly-N-acetyllactosamine-type sugar chains like  band 3, on the polyvinylidene difluoride blotting membrane.	bind
31349	4	6527	7	NULL	NULL	NULL	NULL	lactoferrin	GP		is a type of					glycoprotein	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biochem-(tokyo)_119_4_8743563_s_3	8743563	125I-labeled  human anti-band 3 IgG specifically bound to band 3 glycoprotein and lactoferrin,  a glycoprotein that has poly-N-acetyllactosamine-type sugar chains like  band 3, on the polyvinylidene difluoride blotting membrane.	bind
20526	2	6528	5	NULL	NULL	0	NULL	statement 1	NULL		via	NULL				cell surface	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_41_3_376_s_68	10706585	125I-labeled AcLDL binding   ell surface binding of 125I-labeled AcLDL to MPM was measured as described by Nakagawara and Nathan  ( 33) and Brown et al.  ( 36) Briefly, cells were cultured as described above, in the presence or absence of 10 ng/ml of IL-4 for 96 h.	bind
20527	1	6528	5	NULL	NULL	0	NULL	AcLDL	NULL	125I-labeled	bind	NULL				MPM	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_41_3_376_s_68	10706585	125I-labeled AcLDL binding   ell surface binding of 125I-labeled AcLDL to MPM was measured as described by Nakagawara and Nathan  ( 33) and Brown et al.  ( 36) Briefly, cells were cultured as described above, in the presence or absence of 10 ng/ml of IL-4 for 96 h.	bind
24403	1	6528	7	NULL	NULL	NULL	NULL	AcLDL	GP	125I-labeled	bind					MPM	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_41_3_376_s_68	10706585	125I-labeled AcLDL binding   ell surface binding of 125I-labeled AcLDL to MPM was measured as described by Nakagawara and Nathan  ( 33) and Brown et al.  ( 36) Briefly, cells were cultured as described above, in the presence or absence of 10 ng/ml of IL-4 for 96 h.	bind
31350	2	6528	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs via					cell surface	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_41_3_376_s_68	10706585	125I-labeled AcLDL binding   ell surface binding of 125I-labeled AcLDL to MPM was measured as described by Nakagawara and Nathan  ( 33) and Brown et al.  ( 36) Briefly, cells were cultured as described above, in the presence or absence of 10 ng/ml of IL-4 for 96 h.	bind
20528	1	6529	5	NULL	NULL	0	NULL	ADA	NULL	125I-labeled	bind	NULL				Pg 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_20_20993_s_140	15016824	125I-labeled ADA also binds to Pg 2 electroblotted to a nitrocellulose membrane after electrophoresis ( Fig. 5,  inset, lane 2).	bind
24404	1	6529	7	NULL	NULL	NULL	NULL	ADA	GP	125I-labeled	bind					Pg2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_20_20993_s_140	15016824	125I-labeled ADA also binds to Pg 2 electroblotted to a nitrocellulose membrane after electrophoresis ( Fig. 5,  inset, lane 2).	bind
20529	1	6530	5	NULL	NULL	0	NULL	ankyrin-B	NULL	125I-Labeled	bind	NULL	saturable	C-terminal domain		GST-Hdj1/Hsp40	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_24_25798_s_167	15075330	125I-Labeled ankyrin-B C-terminal domain binds to GST-Hdj1/Hsp40 in a saturable manner with a  K d of 53 nM ( Fig. 6).	bind
24405	1	6530	7	NULL	NULL	NULL	NULL	ankyrin-B	GP	125I-Labeled	bind		saturably	C-terminal domain		GST-Hdj1/Hsp40 	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_24_25798_s_167	15075330	125I-Labeled ankyrin-B C-terminal domain binds to GST-Hdj1/Hsp40 in a saturable manner with a  K d of 53 nM ( Fig. 6).	bind
20530	1	6531	5	NULL	NULL	0	NULL	anti-Tac	NULL	125I-Labeled	bind	NULL				IL-2R/sorLA transfectants	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_25_22788_s_266	11294867	125I-Labeled anti-Tac bound to the IL-2R/sorLA transfectants at 4  degrees C but not to mock transfected cells (not shown).	bind
20531	2	6531	5	NULL	NULL	0	NULL	anti-Tac	NULL	125I-Labeled	does not bind	NULL				mock transfected cells	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_25_22788_s_266	11294867	125I-Labeled anti-Tac bound to the IL-2R/sorLA transfectants at 4  degrees C but not to mock transfected cells (not shown).	bind
24406	1	6531	7	NULL	NULL	NULL	NULL	anti-Tac	GP	125I-Labeled	bind					IL-2R/sorLA transfectants	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_25_22788_s_266	11294867	125I-Labeled anti-Tac bound to the IL-2R/sorLA transfectants at 4  degrees C but not to mock transfected cells (not shown).	bind
24407	2	6531	7	NULL	NULL	NULL	NULL	anti-Tac	GP	125I-labeled	does not bind					mock transfected cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_25_22788_s_266	11294867	125I-Labeled anti-Tac bound to the IL-2R/sorLA transfectants at 4  degrees C but not to mock transfected cells (not shown).	bind
20532	1	6532	5	NULL	NULL	0	NULL	B2	NULL	125I-labeled	bind	NULL	high affinity			TSHR	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_thyroid_15_7_16053383_s_5	16053383	125I-labeled B2 bound to the TSHR with high affinity  (2 x 10(10) L/mol) and patient serum TSHR autoantibodies inhibited labeled  B2 binding to the receptor in a similar way to inhibition of labeled TSH  binding (r = 0.75; n = 20).	bind
20534	2	6532	5	NULL	NULL	0	NULL	TSHR autoantibodies	NULL	patient serum	inhibit	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_thyroid_15_7_16053383_s_5	16053383	125I-labeled B2 bound to the TSHR with high affinity  (2 x 10(10) L/mol) and patient serum TSHR autoantibodies inhibited labeled  B2 binding to the receptor in a similar way to inhibition of labeled TSH  binding (r = 0.75; n = 20).	bind
20535	3	6532	5	NULL	NULL	0	NULL	TSHR autoantibodies	NULL	patient serum	inhibit	NULL				TSH 	NULL	labeled binding of			NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_thyroid_15_7_16053383_s_5	16053383	125I-labeled B2 bound to the TSHR with high affinity  (2 x 10(10) L/mol) and patient serum TSHR autoantibodies inhibited labeled  B2 binding to the receptor in a similar way to inhibition of labeled TSH  binding (r = 0.75; n = 20).	bind
20536	4	6532	5	NULL	NULL	0	NULL	statement 2	NULL		is similar to	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_thyroid_15_7_16053383_s_5	16053383	125I-labeled B2 bound to the TSHR with high affinity  (2 x 10(10) L/mol) and patient serum TSHR autoantibodies inhibited labeled  B2 binding to the receptor in a similar way to inhibition of labeled TSH  binding (r = 0.75; n = 20).	bind
24408	1	6532	7	NULL	NULL	NULL	NULL	B2	GP	125I-labeled	bind		high affinity			TSHR	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_thyroid_15_7_16053383_s_5	16053383	125I-labeled B2 bound to the TSHR with high affinity  (2 x 10(10) L/mol) and patient serum TSHR autoantibodies inhibited labeled  B2 binding to the receptor in a similar way to inhibition of labeled TSH  binding (r = 0.75; n = 20).	bind
24409	2	6532	7	NULL	NULL	NULL	NULL	TSHR autoantibodies 	GP	patient serum	inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_thyroid_15_7_16053383_s_5	16053383	125I-labeled B2 bound to the TSHR with high affinity  (2 x 10(10) L/mol) and patient serum TSHR autoantibodies inhibited labeled  B2 binding to the receptor in a similar way to inhibition of labeled TSH  binding (r = 0.75; n = 20).	bind
24410	3	6532	7	NULL	NULL	NULL	NULL	TSHR autoantibodies	GP	patient serum	inhibits					TSH	GP	binding of			NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_thyroid_15_7_16053383_s_5	16053383	125I-labeled B2 bound to the TSHR with high affinity  (2 x 10(10) L/mol) and patient serum TSHR autoantibodies inhibited labeled  B2 binding to the receptor in a similar way to inhibition of labeled TSH  binding (r = 0.75; n = 20).	bind
24411	4	6532	7	NULL	NULL	NULL	NULL	statement 2	Process		is similar to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_thyroid_15_7_16053383_s_5	16053383	125I-labeled B2 bound to the TSHR with high affinity  (2 x 10(10) L/mol) and patient serum TSHR autoantibodies inhibited labeled  B2 binding to the receptor in a similar way to inhibition of labeled TSH  binding (r = 0.75; n = 20).	bind
20537	1	6533	5	10	NULL	0	NULL	B7 Ig		125I-labeled	bind					CHO cells		CD28-transfected			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-exp-med_173_3_1847722_s_6	1847722	125I-labeled B7 Ig bound to CD28-transfected Chinese  hamster ovary (CHO) cells, and to immobilized CD28 Ig with a Kd approximately  200 nM. B7 Ig also inhibited CD28-mediated cellular adhesion.	bind
20538	2	6533	5	NULL	NULL	0	NULL	CHO cells	NULL		is	NULL				Chinese hamster ovary cells	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-exp-med_173_3_1847722_s_6	1847722	125I-labeled B7 Ig bound to CD28-transfected Chinese  hamster ovary (CHO) cells, and to immobilized CD28 Ig with a Kd approximately  200 nM. B7 Ig also inhibited CD28-mediated cellular adhesion.	bind
20539	3	6533	5	NULL	NULL	0	NULL	B7 Ig	NULL	125I-labeled	bind	NULL				CD28 Ig	NULL	immobilized			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-exp-med_173_3_1847722_s_6	1847722	125I-labeled B7 Ig bound to CD28-transfected Chinese  hamster ovary (CHO) cells, and to immobilized CD28 Ig with a Kd approximately  200 nM. B7 Ig also inhibited CD28-mediated cellular adhesion.	bind
20540	4	6533	5	NULL	NULL	0	NULL	CD28	NULL		mediates	NULL				cellular adhesion	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-exp-med_173_3_1847722_s_6	1847722	125I-labeled B7 Ig bound to CD28-transfected Chinese  hamster ovary (CHO) cells, and to immobilized CD28 Ig with a Kd approximately  200 nM. B7 Ig also inhibited CD28-mediated cellular adhesion.	bind
30271	5	6533	5	NULL	NULL	0	NULL	B7 Ig	NULL		inhibits	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-exp-med_173_3_1847722_s_6	1847722	125I-labeled B7 Ig bound to CD28-transfected Chinese  hamster ovary (CHO) cells, and to immobilized CD28 Ig with a Kd approximately  200 nM. B7 Ig also inhibited CD28-mediated cellular adhesion.	bind
24413	1	6533	7	NULL	NULL	NULL	NULL	 B7 Ig 	GP	125I-labeled	binds to					CHO cells	Cell	CD28-transfected			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-exp-med_173_3_1847722_s_6	1847722	125I-labeled B7 Ig bound to CD28-transfected Chinese  hamster ovary (CHO) cells, and to immobilized CD28 Ig with a Kd approximately  200 nM. B7 Ig also inhibited CD28-mediated cellular adhesion.	bind
24414	2	6533	7	NULL	NULL	NULL	NULL	B7 Ig	GP	125I-labeled	binds to					CD28 Ig 	GP	immobilized			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-exp-med_173_3_1847722_s_6	1847722	125I-labeled B7 Ig bound to CD28-transfected Chinese  hamster ovary (CHO) cells, and to immobilized CD28 Ig with a Kd approximately  200 nM. B7 Ig also inhibited CD28-mediated cellular adhesion.	bind
24415	3	6533	7	NULL	NULL	NULL	NULL	CD28	Cell		mediates					cellular adhesion	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-exp-med_173_3_1847722_s_6	1847722	125I-labeled B7 Ig bound to CD28-transfected Chinese  hamster ovary (CHO) cells, and to immobilized CD28 Ig with a Kd approximately  200 nM. B7 Ig also inhibited CD28-mediated cellular adhesion.	bind
24416	4	6533	7	NULL	NULL	NULL	NULL	B7 Ig	GP		inhibits					statement 3	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-exp-med_173_3_1847722_s_6	1847722	125I-labeled B7 Ig bound to CD28-transfected Chinese  hamster ovary (CHO) cells, and to immobilized CD28 Ig with a Kd approximately  200 nM. B7 Ig also inhibited CD28-mediated cellular adhesion.	bind
31351	5	6533	7	NULL	NULL	NULL	NULL	CHO	Cell		is					Chinese hamster ovary cells	Cell				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-exp-med_173_3_1847722_s_6	1847722	125I-labeled B7 Ig bound to CD28-transfected Chinese  hamster ovary (CHO) cells, and to immobilized CD28 Ig with a Kd approximately  200 nM. B7 Ig also inhibited CD28-mediated cellular adhesion.	bind
20541	1	6534	5	NULL	NULL	0	NULL	beta-glucuronidase	NULL	125I-Labeled	bind	NULL	specifically			IGF-IIPRs	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_35_22358_s_209	9712856	125I-Labeled beta-glucuronidase specifically bound to the IGF-IIPRs was eluted by incubation for 1 h with 10 mM Man-6-P.	bind
24419	1	6534	7	NULL	NULL	NULL	NULL	beta-glucuronidase	GP	125I-Labeled 	bind		specifically			IGF-IIPRs	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_35_22358_s_209	9712856	125I-Labeled beta-glucuronidase specifically bound to the IGF-IIPRs was eluted by incubation for 1 h with 10 mM Man-6-P.	bind
20542	1	6535	5	NULL	NULL	0	NULL	BMP-7	NULL	125I-Labeled	bind	NULL				ROS 17/2	NULL				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_308_4_858_s_200	12927798	125I-Labeled BMP-7 binding to ROS 17/2.	bind
24420	1	6535	7	NULL	NULL	NULL	NULL	BMP-7	GP	125I-Labeled	binds to					ROS 17/2	Cell				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_308_4_858_s_200	12927798	125I-Labeled BMP-7 binding to ROS 17/2.	bind
20585	1	6536	5	10	NULL	0	NULL	HEK 293T cells	NULL	intact	express	NULL	transiently			GnRH-R constructs	NULL	wt;; catfish			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_56_6_1229_s_174	10570050	125I-Labeled cGnRH-II binding to intact HEK 293T cells transiently expressing wt or Ser-mutant catfish GnRH-R constructs was performed in the presence or absence of 10 6 M unlabeled cGnRH-II.	bind
20586	2	6536	5	10	NULL	0	NULL	HEK 293T cells	NULL	intact	express	NULL	transiently			GnRH-R constructs	NULL	mutant;; catfish	Ser		NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_56_6_1229_s_174	10570050	125I-Labeled cGnRH-II binding to intact HEK 293T cells transiently expressing wt or Ser-mutant catfish GnRH-R constructs was performed in the presence or absence of 10 6 M unlabeled cGnRH-II.	bind
20587	3	6536	5	NULL	NULL	0	NULL	cGnRH-II	NULL	125I-Labeled	bind	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_56_6_1229_s_174	10570050	125I-Labeled cGnRH-II binding to intact HEK 293T cells transiently expressing wt or Ser-mutant catfish GnRH-R constructs was performed in the presence or absence of 10 6 M unlabeled cGnRH-II.	bind
20588	4	6536	5	NULL	NULL	0	NULL	cGnRH-II	NULL	125I-Labeled	bind	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_56_6_1229_s_174	10570050	125I-Labeled cGnRH-II binding to intact HEK 293T cells transiently expressing wt or Ser-mutant catfish GnRH-R constructs was performed in the presence or absence of 10 6 M unlabeled cGnRH-II.	bind
20589	5	6536	5	NULL	NULL	0	NULL	statement 3	NULL		is an alternative to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_56_6_1229_s_174	10570050	125I-Labeled cGnRH-II binding to intact HEK 293T cells transiently expressing wt or Ser-mutant catfish GnRH-R constructs was performed in the presence or absence of 10 6 M unlabeled cGnRH-II.	bind
24476	1	6536	7	NULL	NULL	NULL	NULL	HEK 293T cells 	Cell	intact	express		transiently			GnRH-R constructs	GP	wt;; catfish			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_56_6_1229_s_174	10570050	125I-Labeled cGnRH-II binding to intact HEK 293T cells transiently expressing wt or Ser-mutant catfish GnRH-R constructs was performed in the presence or absence of 10 6 M unlabeled cGnRH-II.	bind
24477	2	6536	7	NULL	NULL	NULL	NULL	HEK 293T cells 	Cell	intact	express		transiently			GnRH-R constructs	GP	mutant;; catfish	Ser		NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_56_6_1229_s_174	10570050	125I-Labeled cGnRH-II binding to intact HEK 293T cells transiently expressing wt or Ser-mutant catfish GnRH-R constructs was performed in the presence or absence of 10 6 M unlabeled cGnRH-II.	bind
24478	3	6536	7	NULL	NULL	NULL	NULL	 cGnRH-II	GP	125I-Labeled	bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_56_6_1229_s_174	10570050	125I-Labeled cGnRH-II binding to intact HEK 293T cells transiently expressing wt or Ser-mutant catfish GnRH-R constructs was performed in the presence or absence of 10 6 M unlabeled cGnRH-II.	bind
24479	4	6536	7	NULL	NULL	NULL	NULL	cGnRH-II	GP	125I-labeled	bind					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_56_6_1229_s_174	10570050	125I-Labeled cGnRH-II binding to intact HEK 293T cells transiently expressing wt or Ser-mutant catfish GnRH-R constructs was performed in the presence or absence of 10 6 M unlabeled cGnRH-II.	bind
24480	5	6536	7	NULL	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_56_6_1229_s_174	10570050	125I-Labeled cGnRH-II binding to intact HEK 293T cells transiently expressing wt or Ser-mutant catfish GnRH-R constructs was performed in the presence or absence of 10 6 M unlabeled cGnRH-II.	bind
20574	1	6537	5	NULL	NULL	0	NULL	Cry1Ac	NULL	125I-labeled	bind	NULL	specifically			brush border membrane vesicles	NULL	E. insulana			NULL		0	NULL	NULL	NULL	abs-batch0580-0599_appl-environ-microbiol_72_1_16391075_s_12	16391075	125I-labeled Cry1Ac and Cry1Ab and biotinylated Cry1Ba,  Cry1Ia, and Cry9Ca showed specific binding to the brush border membrane  vesicles from E. insulana.	bind
20575	2	6537	5	NULL	NULL	0	NULL	Cry1Ab	NULL	125I-labeled	bind	NULL	specifically			brush border membrane vesicles	NULL	E. insulana			NULL		0	NULL	NULL	NULL	abs-batch0580-0599_appl-environ-microbiol_72_1_16391075_s_12	16391075	125I-labeled Cry1Ac and Cry1Ab and biotinylated Cry1Ba,  Cry1Ia, and Cry9Ca showed specific binding to the brush border membrane  vesicles from E. insulana.	bind
20576	3	6537	5	NULL	NULL	0	NULL	Cry1Ba	NULL	biotinylated	bind	NULL	specifically			brush border membrane vesicles	NULL	E. insulana			NULL		0	NULL	NULL	NULL	abs-batch0580-0599_appl-environ-microbiol_72_1_16391075_s_12	16391075	125I-labeled Cry1Ac and Cry1Ab and biotinylated Cry1Ba,  Cry1Ia, and Cry9Ca showed specific binding to the brush border membrane  vesicles from E. insulana.	bind
20577	4	6537	5	NULL	NULL	0	NULL	Cry1Ia	NULL	biotinylated	bind	NULL	specifically			brush border membrane vesicles	NULL	E. insulana			NULL		0	NULL	NULL	NULL	abs-batch0580-0599_appl-environ-microbiol_72_1_16391075_s_12	16391075	125I-labeled Cry1Ac and Cry1Ab and biotinylated Cry1Ba,  Cry1Ia, and Cry9Ca showed specific binding to the brush border membrane  vesicles from E. insulana.	bind
20578	5	6537	5	NULL	NULL	0	NULL	Cry9Ca	NULL	biotinylated	bind	NULL	specifically			brush border membrane vesicles	NULL	E. insulana			NULL		0	NULL	NULL	NULL	abs-batch0580-0599_appl-environ-microbiol_72_1_16391075_s_12	16391075	125I-labeled Cry1Ac and Cry1Ab and biotinylated Cry1Ba,  Cry1Ia, and Cry9Ca showed specific binding to the brush border membrane  vesicles from E. insulana.	bind
24481	1	6537	7	NULL	NULL	NULL	NULL	Cry1Ac 	GP	125I-labeled 	bind		specific			 brush border membrane vesicles	CellComponent	E. insulana			NULL		NULL	NULL	NULL	NULL	abs-batch0580-0599_appl-environ-microbiol_72_1_16391075_s_12	16391075	125I-labeled Cry1Ac and Cry1Ab and biotinylated Cry1Ba,  Cry1Ia, and Cry9Ca showed specific binding to the brush border membrane  vesicles from E. insulana.	bind
24482	2	6537	7	NULL	NULL	NULL	NULL	Cry1Ab	GP	125I-labeled	bind		specific			brush border membrane vesicles	CellComponent	E. insulana			NULL		NULL	NULL	NULL	NULL	abs-batch0580-0599_appl-environ-microbiol_72_1_16391075_s_12	16391075	125I-labeled Cry1Ac and Cry1Ab and biotinylated Cry1Ba,  Cry1Ia, and Cry9Ca showed specific binding to the brush border membrane  vesicles from E. insulana.	bind
24483	3	6537	7	NULL	NULL	NULL	NULL	Cry1Ba	GP	biotinylated	bind		specific			brush border membrane vesicles	CellComponent	E.insulana			NULL		NULL	NULL	NULL	NULL	abs-batch0580-0599_appl-environ-microbiol_72_1_16391075_s_12	16391075	125I-labeled Cry1Ac and Cry1Ab and biotinylated Cry1Ba,  Cry1Ia, and Cry9Ca showed specific binding to the brush border membrane  vesicles from E. insulana.	bind
24484	4	6537	7	NULL	NULL	NULL	NULL	Cry1Ia	GP	biotinylated	bind		specific			brush border membrane vesicles	CellComponent	E.insulana			NULL		NULL	NULL	NULL	NULL	abs-batch0580-0599_appl-environ-microbiol_72_1_16391075_s_12	16391075	125I-labeled Cry1Ac and Cry1Ab and biotinylated Cry1Ba,  Cry1Ia, and Cry9Ca showed specific binding to the brush border membrane  vesicles from E. insulana.	bind
24485	5	6537	7	NULL	NULL	NULL	NULL	Cry9Ca	GP	biotinylated	bind		specific			brush border membrane vesicles	CellComponent	E.insulana			NULL		NULL	NULL	NULL	NULL	abs-batch0580-0599_appl-environ-microbiol_72_1_16391075_s_12	16391075	125I-labeled Cry1Ac and Cry1Ab and biotinylated Cry1Ba,  Cry1Ia, and Cry9Ca showed specific binding to the brush border membrane  vesicles from E. insulana.	bind
20634	1	6538	5	NULL	NULL	0	NULL	Cry1Ab	NULL	125I-labeled	bind	NULL	specifically			brush border membrane vesicles	NULL	E. insulana			NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_1_437_s_12	16391075	125I-labeled Cry1Ac and Cry1Ab and biotinylated Cry1Ba, Cry1Ia, and Cry9Ca showed specific binding to the brush border membrane vesicles from  E. insulana.	bind
20635	2	6538	5	NULL	NULL	0	NULL	Cry1Ac	NULL	125I-labeled	bind	NULL	specifically			brush border membrane vesicles	NULL	E. insulana			NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_1_437_s_12	16391075	125I-labeled Cry1Ac and Cry1Ab and biotinylated Cry1Ba, Cry1Ia, and Cry9Ca showed specific binding to the brush border membrane vesicles from  E. insulana.	bind
20636	3	6538	5	NULL	NULL	0	NULL	Cry1Ba	NULL	biotinylated	bind	NULL	specifically			brush border membrane vesicles	NULL	E. insulana			NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_1_437_s_12	16391075	125I-labeled Cry1Ac and Cry1Ab and biotinylated Cry1Ba, Cry1Ia, and Cry9Ca showed specific binding to the brush border membrane vesicles from  E. insulana.	bind
20637	4	6538	5	NULL	NULL	0	NULL	Cry1Ia	NULL	biotinylated	bind	NULL	specifically			brush border membrane vesicles	NULL	E. insulana			NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_1_437_s_12	16391075	125I-labeled Cry1Ac and Cry1Ab and biotinylated Cry1Ba, Cry1Ia, and Cry9Ca showed specific binding to the brush border membrane vesicles from  E. insulana.	bind
20638	5	6538	5	NULL	NULL	0	NULL	Cry9Ca	NULL	biotinylated	bind	NULL	specifically			brush border membrane vesicles	NULL	E. insulana			NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_1_437_s_12	16391075	125I-labeled Cry1Ac and Cry1Ab and biotinylated Cry1Ba, Cry1Ia, and Cry9Ca showed specific binding to the brush border membrane vesicles from  E. insulana.	bind
20580	1	6539	5	NULL	NULL	0	NULL	DNT1-54	NULL	125I-labeled	bind	NULL				MC3T3-E1	NULL	DNT-susceptible			NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
20581	2	6539	5	NULL	NULL	0	NULL	DNT1-54	NULL	125I-labeled	bind	NULL				C3H10T1/2	NULL	DNT-susceptible			NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
20582	3	6539	5	NULL	NULL	0	NULL	DNT1-54	NULL	125I-labeled	bind	NULL				Swiss 3T3	NULL	DNT-susceptible			NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
20583	4	6539	5	NULL	NULL	0	NULL	DNT1-54	NULL	125I-labeled	bind	NULL				rat embryo fibroblasts	NULL	DNT-susceptible			NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
20584	5	6539	5	NULL	NULL	0	NULL	DNT1-54	NULL	125I-labeled	bind	NULL				NIH 3T3 cells	NULL	DNT-susceptible			NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
20639	6	6539	5	NULL	NULL	0	NULL	DNT1-54	NULL	125I-labeled	does not bind	NULL				COS7 cells	NULL	resistant			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
20640	7	6539	5	NULL	NULL	0	NULL	DNT1-54	NULL	125I-labeled	does not bind	NULL				BALB/3T3 cells	NULL	resistant			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
20641	8	6539	5	NULL	NULL	0	NULL	DNT1-54	NULL	125I-labeled	does not bind	NULL				L929 cells	NULL	resistant			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
20642	9	6539	5	NULL	NULL	0	NULL	DNT1-54	NULL	125I-labeled	does not bind	NULL				PAE cells	NULL	resistant			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
20643	10	6539	5	NULL	NULL	0	NULL	DNT1-54	NULL	125I-labeled	does not bind	NULL				K562 cells	NULL	resistant			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
20644	11	6539	5	NULL	NULL	0	NULL	sensitivity of cells	NULL	to DNT	is attributable to	NULL				unknown receptor	NULL	existence of			NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
24486	1	6539	7	NULL	NULL	NULL	NULL	DNT1-54 	GP	125I-labeled	bind					MC3T3-E1 cells	Cell	 DNT-susceptible			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
24487	2	6539	7	NULL	NULL	NULL	NULL	DNT1-54 	GP	125I-labeled	bind					C3H10T1/2 cells	Cell	DNT-susceptible			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
24488	3	6539	7	NULL	NULL	NULL	NULL	DNT1-54 	GP	125I-labeled	bind					Swiss 3T3 cells	Cell	DNT-susceptible			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
24489	4	6539	7	NULL	NULL	NULL	NULL	DNT1-54	GP	125I-labeled	bind					embryo fibroblasts	Cell	DNT-susceptible rat 			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
24490	5	6539	7	NULL	NULL	NULL	NULL	DNT1-54	GP	125I-labeled	bind					NIH 3T3 cells 	Cell	DNT-susceptible			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
24491	6	6539	7	NULL	NULL	NULL	NULL	DNT1-54 	GP	125I-labeled	does not bind					COS7 cells	Cell	DNT-resistant			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
24492	7	6539	7	NULL	NULL	NULL	NULL	DNT1-54	GP	125I-labeled	does not bind					BALB/3T3 cells	Cell	DNT-resistant			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
24493	8	6539	7	NULL	NULL	NULL	NULL	DNT1-54	GP	125I-labeled	does not bind					L929 cells	Cell	DNT-resistant			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
24494	9	6539	7	NULL	NULL	NULL	NULL	DNT1-54	GP	125I-labeled 	does not bind					PAE cells	Cell	DNT-resistant			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
24495	10	6539	7	NULL	NULL	NULL	NULL	DNT1-54	GP	125I-labeled	does not bind					K562 cells	Cell	DNT-resistant			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
24496	11	6539	7	NULL	NULL	NULL	NULL	statement 1	Process	DNT sensitivity in	indicate					unknown receptor	GP	existence of			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
24497	12	6539	7	NULL	NULL	NULL	NULL	statement 2	Process	DNT sensitivity in	indicate					unknown receptor	GP	existence of			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
24498	13	6539	7	NULL	NULL	NULL	NULL	statement 3	Process	DNT sensitivity in	indicate					unknown receptor	GP	existence of			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
24500	14	6539	7	NULL	NULL	NULL	NULL	statement 4	Process	DNT sensitivity in	indicate					unknown receptor	GP	existence of			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
31399	15	6539	7	NULL	NULL	NULL	NULL	statement 5	Process	DNT sensitivity in	indicate					unknown receptor	GP	existence of			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
31400	16	6539	7	NULL	NULL	NULL	NULL	statement 6	Process	DNT sensitivity in	indicate					unknown receptor	GP	existence of			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
31401	17	6539	7	NULL	NULL	NULL	NULL	statement 7	Process	DNT sensitivity in	indicate					unknown receptor	GP	existence of			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
31402	18	6539	7	NULL	NULL	NULL	NULL	statement 8	Process	DNT sensitivity in	indicate					unknown receptor	GP	existence of			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
31403	19	6539	7	NULL	NULL	NULL	NULL	statement 9	Process	DNT sensitivity in	indicate					unknown receptor	GP	existence of			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
31404	20	6539	7	NULL	NULL	NULL	NULL	statement 10	Process	DNT sensitivity in	indicate					unknown receptor	GP	existence of			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3427_s_160	12065482	125I-labeled DNT1-54 bound to the DNT-susceptible MC3T3-E1, C3H10T1/2, Swiss 3T3, rat embryo fibroblasts, and NIH 3T3 cells but not to the resistant COS7, BALB/3T3, L929, PAE, and K562 cells (Fig.  4D), indicating that the sensitivity of cells to DNT is attributable to the existence of an unknown receptor.	bind
20645	1	6540	5	NULL	NULL	0	NULL	flagellin	NULL	125I-labeled	bind	NULL				GM1	NULL	glycolipid			NULL	in vitro	0	NULL	NULL	NULL	gw60_infectimmun_66_1_43_s_9	9423837	125I-labeled flagellin bound to the glycolipids GM1 and GD1a and to asialoGM1 in an in vitro binding assay.	bind
20646	2	6540	5	NULL	NULL	0	NULL	flagellin	NULL	125I-labeled	bind	NULL				GD1a	NULL	glycolipid			NULL	in vitro	0	NULL	NULL	NULL	gw60_infectimmun_66_1_43_s_9	9423837	125I-labeled flagellin bound to the glycolipids GM1 and GD1a and to asialoGM1 in an in vitro binding assay.	bind
20647	3	6540	5	NULL	NULL	0	NULL	flagellin	NULL	125I-labeled	bind	NULL				asialoGM1	NULL	glycolipid			NULL	in vitro	0	NULL	NULL	NULL	gw60_infectimmun_66_1_43_s_9	9423837	125I-labeled flagellin bound to the glycolipids GM1 and GD1a and to asialoGM1 in an in vitro binding assay.	bind
24501	1	6540	7	NULL	NULL	NULL	NULL	flagellin	GP	125I-labeled	bind					GM1	Chemical	glycolipids			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_infectimmun_66_1_43_s_9	9423837	125I-labeled flagellin bound to the glycolipids GM1 and GD1a and to asialoGM1 in an in vitro binding assay.	bind
24502	2	6540	7	NULL	NULL	NULL	NULL	flagellin	GP	125I-labeled	bind					GD1a	Chemical	glycolipids			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_infectimmun_66_1_43_s_9	9423837	125I-labeled flagellin bound to the glycolipids GM1 and GD1a and to asialoGM1 in an in vitro binding assay.	bind
24503	3	6540	7	NULL	NULL	NULL	NULL	flagellin	GP	125I-labeled	bind					asialoGM1	Chemical	glycolipids			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_infectimmun_66_1_43_s_9	9423837	125I-labeled flagellin bound to the glycolipids GM1 and GD1a and to asialoGM1 in an in vitro binding assay.	bind
20649	1	6542	5	10	NULL	0	NULL	galanin		125I-labeled;;human	bind		saturably			GalR2 receptor		rat			NULL	COS-1 cells	NULL	NULL	NULL	NULL	gw60_molpharmacol_52_3_337_s_8	9281594	125I-Labeled human galanin binding to rat GalR2 receptor expressed in COS-1 cells was saturable ( Kd = 0.59 nM) and could be displaced by galanin, several galanin fragments, and chimeric peptides.	bind
20650	2	6542	5	NULL	NULL	0	NULL	galanin	NULL		displace	NULL				statement 1	NULL	ligand of			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_52_3_337_s_8	9281594	125I-Labeled human galanin binding to rat GalR2 receptor expressed in COS-1 cells was saturable ( Kd = 0.59 nM) and could be displaced by galanin, several galanin fragments, and chimeric peptides.	bind
20651	4	6542	5	NULL	NULL	0	NULL	several galanin fragments	NULL		displace	NULL				statement 1	NULL	ligand of			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_52_3_337_s_8	9281594	125I-Labeled human galanin binding to rat GalR2 receptor expressed in COS-1 cells was saturable ( Kd = 0.59 nM) and could be displaced by galanin, several galanin fragments, and chimeric peptides.	bind
20652	5	6542	5	NULL	NULL	0	NULL	chimeric peptides	NULL		displace	NULL				statement 1	NULL	ligand of			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_52_3_337_s_8	9281594	125I-Labeled human galanin binding to rat GalR2 receptor expressed in COS-1 cells was saturable ( Kd = 0.59 nM) and could be displaced by galanin, several galanin fragments, and chimeric peptides.	bind
24504	1	6542	7	NULL	NULL	NULL	NULL	galanin	GP	125I-labeled;;human	binds to		saturably			GalR2 receptor	GP	rat			NULL	COS-1 cells	NULL	NULL	NULL	NULL	gw60_molpharmacol_52_3_337_s_8	9281594	125I-Labeled human galanin binding to rat GalR2 receptor expressed in COS-1 cells was saturable ( Kd = 0.59 nM) and could be displaced by galanin, several galanin fragments, and chimeric peptides.	bind
24506	2	6542	7	NULL	NULL	NULL	NULL	galanin	GP		displace					statement 1	Process	ligand of			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_52_3_337_s_8	9281594	125I-Labeled human galanin binding to rat GalR2 receptor expressed in COS-1 cells was saturable ( Kd = 0.59 nM) and could be displaced by galanin, several galanin fragments, and chimeric peptides.	bind
24507	3	6542	7	NULL	NULL	NULL	NULL	galanin fragments	AminoAcid		displace					statement 1	Process	ligand of			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_52_3_337_s_8	9281594	125I-Labeled human galanin binding to rat GalR2 receptor expressed in COS-1 cells was saturable ( Kd = 0.59 nM) and could be displaced by galanin, several galanin fragments, and chimeric peptides.	bind
31405	4	6542	7	NULL	NULL	NULL	NULL	galanin	GP	chimeric peptides	displace 					statement 1	Process	ligand of			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_52_3_337_s_8	9281594	125I-Labeled human galanin binding to rat GalR2 receptor expressed in COS-1 cells was saturable ( Kd = 0.59 nM) and could be displaced by galanin, several galanin fragments, and chimeric peptides.	bind
20653	1	6543	5	10	NULL	0	NULL	NPW23		125I-labeled;;human	bind					GPR7		human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_39_35826_s_178	12130646	125I-Labeled human NPW23 bound both human GPR7 and GPR8 with nearly the same affinity.	bind
20654	2	6543	5	10	NULL	0	NULL	NPW23		125I-labeled;;human	bind					GPR8		human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_39_35826_s_178	12130646	125I-Labeled human NPW23 bound both human GPR7 and GPR8 with nearly the same affinity.	bind
20655	3	6543	5	NULL	NULL	0	NULL	statement 1	NULL		same affinity as	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_39_35826_s_178	12130646	125I-Labeled human NPW23 bound both human GPR7 and GPR8 with nearly the same affinity.	bind
24508	1	6543	7	NULL	NULL	NULL	NULL	NPW23	GP	125I-labeled;;human	bind					GPR7	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_39_35826_s_178	12130646	125I-Labeled human NPW23 bound both human GPR7 and GPR8 with nearly the same affinity.	bind
24509	2	6543	7	NULL	NULL	NULL	NULL	 NPW23	GP	125I-labeled;;human	bind					GPR8	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_39_35826_s_178	12130646	125I-Labeled human NPW23 bound both human GPR7 and GPR8 with nearly the same affinity.	bind
24510	3	6543	7	NULL	NULL	NULL	NULL	statement 1	Process		same affinity as					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_39_35826_s_178	12130646	125I-Labeled human NPW23 bound both human GPR7 and GPR8 with nearly the same affinity.	bind
20656	1	6544	5	NULL	NULL	0	NULL	JRFL gp120	NULL	125I-labeled	bind	NULL				HEK-293 cells	NULL	CCR5-transiently transfected			NULL		0	NULL	NULL	NULL	gw60_pnas_97_7_3388_s_43	10725362	125I-labeled JRFL gp120 was allowed to bind to CCR5-transiently transfected HEK-293 cells in Hepes binding buffer (50 nM Hepes, pH 7.4/5 nM MgCl2) with 0.5% BSA, alone or with 2D7 mAb ( 20), CCR5-02, or mIg.	bind
24511	1	6544	7	NULL	NULL	NULL	NULL	JRFL gp120	GP	125I-labeled	bind					HEK-293 cells	Cell	CCR5-transiently transfected			NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_7_3388_s_43	10725362	125I-labeled JRFL gp120 was allowed to bind to CCR5-transiently transfected HEK-293 cells in Hepes binding buffer (50 nM Hepes, pH 7.4/5 nM MgCl2) with 0.5% BSA, alone or with 2D7 mAb ( 20), CCR5-02, or mIg.	bind
20657	1	6546	5	NULL	NULL	0	NULL	MMP-9	NULL	125I-labeled	bind	NULL	specifically	C-domain		CS-1 melanoma cells	NULL	beta5 integrin-transfected			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_28_29589_s_296	15123665	125I-Labeled MMP-9 C domain showed a specific binding to beta5 integrin-transfected, but not to the untransfected CS-1 melanoma cells ( Fig. 6 A).	bind
20658	2	6546	5	10	NULL	0	NULL	MMP-9		125I-labeled	does not bind			C domain		CS-1 melanoma cells		untransfected			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_28_29589_s_296	15123665	125I-Labeled MMP-9 C domain showed a specific binding to beta5 integrin-transfected, but not to the untransfected CS-1 melanoma cells ( Fig. 6 A).	bind
24512	1	6546	7	NULL	NULL	NULL	NULL	MMP-9 	GP	125I-Labeled	bind		specific	C domain		CS-1 melanoma cells	Cell	beta5 integrin-transfected			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_28_29589_s_296	15123665	125I-Labeled MMP-9 C domain showed a specific binding to beta5 integrin-transfected, but not to the untransfected CS-1 melanoma cells ( Fig. 6 A).	bind
24513	2	6546	7	NULL	NULL	NULL	NULL	MMP-9	GP	125I-labeled	does not bind			C domain		CS-1 melanoma cells	Cell	untransfected			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_28_29589_s_296	15123665	125I-Labeled MMP-9 C domain showed a specific binding to beta5 integrin-transfected, but not to the untransfected CS-1 melanoma cells ( Fig. 6 A).	bind
20659	1	6547	5	NULL	NULL	0	NULL	neuroserpin	NULL	125I-labeled	bind	NULL	most effectively			LRP	NULL	purified			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_50_50250_s_116	14522960	125I-Labeled neuroserpin binds most effectively to purified LRP after incubation with  tPA.	bind
20660	2	6547	5	NULL	NULL	0	NULL	tPA	NULL	incubation with	is required for	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_50_50250_s_116	14522960	125I-Labeled neuroserpin binds most effectively to purified LRP after incubation with  tPA.	bind
24514	1	6547	7	NULL	NULL	NULL	NULL	neuroserpin	GP	125I-Labeled	binds		effectively			LRP	GP	purified			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_50_50250_s_116	14522960	125I-Labeled neuroserpin binds most effectively to purified LRP after incubation with  tPA.	bind
24515	2	6547	7	NULL	NULL	NULL	NULL	statement 1	Process		occurs after					tPA	GP	incubation with			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_50_50250_s_116	14522960	125I-Labeled neuroserpin binds most effectively to purified LRP after incubation with  tPA.	bind
20661	1	6548	5	NULL	NULL	0	NULL	plasminogen	NULL	125I-labeled	does not bind	NULL				ATP synthase	NULL	recombinant	alpha-subunit 		NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_6_2811_s_179	10077593	125I-labeled plasminogen did not bind to the recombinant alpha-subunit ATP synthase (Fig.  7 E), but did bind to annexin II (Fig.  3 D).	bind
20662	2	6548	5	NULL	NULL	0	NULL	plasminogen	NULL	125I-labeled	bind	NULL				annexin II	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_96_6_2811_s_179	10077593	125I-labeled plasminogen did not bind to the recombinant alpha-subunit ATP synthase (Fig.  7 E), but did bind to annexin II (Fig.  3 D).	bind
24516	1	6548	7	NULL	NULL	NULL	NULL	plasminogen	GP	125I-labeled	does not bind					ATP synthase	GP	recombinant	alpha-subunit		NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_6_2811_s_179	10077593	125I-labeled plasminogen did not bind to the recombinant alpha-subunit ATP synthase (Fig.  7 E), but did bind to annexin II (Fig.  3 D).	bind
24517	2	6548	7	NULL	NULL	NULL	NULL	plasminogen	GP	125I-labeled	bind					annexin II 	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_6_2811_s_179	10077593	125I-labeled plasminogen did not bind to the recombinant alpha-subunit ATP synthase (Fig.  7 E), but did bind to annexin II (Fig.  3 D).	bind
20663	1	6549	5	NULL	NULL	0	NULL	plasminogen	NULL	125I-labeled	does not bind	NULL				p63	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_43_42679_s_199	12913003	125I-labeled plasminogen did not detect isolated p63 in ligand blotting experiments, and p63 did not bind to a plasminogen affinity matrix as detected either by immunoblotting or ligand blotting, although the plasminogen binding protein alpha-enolase ( ) was readily detected by both methods (data not shown).	bind
20664	2	6549	5	NULL	NULL	0	NULL	plasminogen	NULL	125I-labeled	bind	NULL				alpha-enolase	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_43_42679_s_199	12913003	125I-labeled plasminogen did not detect isolated p63 in ligand blotting experiments, and p63 did not bind to a plasminogen affinity matrix as detected either by immunoblotting or ligand blotting, although the plasminogen binding protein alpha-enolase ( ) was readily detected by both methods (data not shown).	bind
24519	1	6549	7	NULL	NULL	NULL	NULL	p63	GP		does not bind					plasminogen 	GP	125I-labeled			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_43_42679_s_199	12913003	125I-labeled plasminogen did not detect isolated p63 in ligand blotting experiments, and p63 did not bind to a plasminogen affinity matrix as detected either by immunoblotting or ligand blotting, although the plasminogen binding protein alpha-enolase ( ) was readily detected by both methods (data not shown).	bind
31406	2	6549	7	NULL	NULL	NULL	NULL	plasminogen	GP	125I-labeled	bind					alpha-enolase	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_43_42679_s_199	12913003	125I-labeled plasminogen did not detect isolated p63 in ligand blotting experiments, and p63 did not bind to a plasminogen affinity matrix as detected either by immunoblotting or ligand blotting, although the plasminogen binding protein alpha-enolase ( ) was readily detected by both methods (data not shown).	bind
20665	1	6550	5	NULL	NULL	0	NULL	protein A	NULL	125I-labeled	bind	NULL				anti-phosphotyrosine antibodies	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_3_992_s_37	15240146	125I-labeled protein A bound to the anti-phosphotyrosine and anti-peptide antibodies  was detected by autoradiography using preflashed Kodak XAR film with Cronex Lightning  Plus intensifying screens at  80  degrees C for 12-48 h.	bind
20666	2	6550	5	NULL	NULL	0	NULL	protein A	NULL	125I-labeled	bind	NULL				anti-peptide antibodies	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_3_992_s_37	15240146	125I-labeled protein A bound to the anti-phosphotyrosine and anti-peptide antibodies  was detected by autoradiography using preflashed Kodak XAR film with Cronex Lightning  Plus intensifying screens at  80  degrees C for 12-48 h.	bind
24522	1	6550	7	NULL	NULL	NULL	NULL	protein A	GP	125I-labeled	bind					anti-phosphotyrosine antibody	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_3_992_s_37	15240146	125I-labeled protein A bound to the anti-phosphotyrosine and anti-peptide antibodies  was detected by autoradiography using preflashed Kodak XAR film with Cronex Lightning  Plus intensifying screens at  80  degrees C for 12-48 h.	bind
24523	2	6550	7	NULL	NULL	NULL	NULL	protein A	GP	125I-labeled	bind					anti-peptide antibodies	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_3_992_s_37	15240146	125I-labeled protein A bound to the anti-phosphotyrosine and anti-peptide antibodies  was detected by autoradiography using preflashed Kodak XAR film with Cronex Lightning  Plus intensifying screens at  80  degrees C for 12-48 h.	bind
20672	1	6553	5	NULL	NULL	0	NULL	SecA	NULL	125I-labeled	bind	NULL				IMVs	NULL	urea-washed			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_8_2243_s_167	11914356	125I-labeled SecA (2 mug) was bound to 4 M urea-washed IMVs (5 mug of proteins in a final volume of 200 mul) at 0 degrees C for 30 min, and the complexes were isolated by centrifugation.	bind
24952	1	6553	7	NULL	NULL	NULL	NULL	SecA	GP	25I-labeled	bind					IMVs	CellComponent	urea washed			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_8_2243_s_167	11914356	125I-labeled SecA (2 mug) was bound to 4 M urea-washed IMVs (5 mug of proteins in a final volume of 200 mul) at 0 degrees C for 30 min, and the complexes were isolated by centrifugation.	bind
20673	1	6556	5	NULL	NULL	0	NULL	VEGF	NULL	125I-labeled	bind	NULL				NRP1	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_25_13_3045_s_278	16763549	125I-labeled VEGF binding to NRP1	bind
24959	1	6556	7	NULL	NULL	NULL	NULL	VEGF	GP	125I-labeled	binds to					NRP1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_13_3045_s_278	16763549	125I-labeled VEGF binding to NRP1	bind
20674	1	6557	5	NULL	NULL	0	NULL	S8-SP11	NULL	125I-labeled	bind	NULL	specifically			S8 homozygote stigmatic microsomal membranes	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nature_413_6855_534_s_50	11586363	125I-labelled  S8-SP11 specifically binds the stigmatic microsomal membranes of the  S8 homozygote ( Fig. 3a).	bind
24962	1	6557	7	NULL	NULL	NULL	NULL	S8-SP11	GP	125I-labelled 	binds		specifically			S8 homozygote stigmatic microsomal membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_nature_413_6855_534_s_50	11586363	125I-labelled  S8-SP11 specifically binds the stigmatic microsomal membranes of the  S8 homozygote ( Fig. 3a).	bind
20675	1	6558	5	NULL	NULL	0	NULL	PK2	NULL		bind	NULL				PK-Rs	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1579_2_173_s_104	12427552	125I-labelled PK2 was used to determine the binding affinity of PK2 for two PK-Rs.	bind
24969	1	6558	7	NULL	NULL	NULL	NULL	PK2	GP		bind					PK-Rs	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1579_2_173_s_104	12427552	125I-labelled PK2 was used to determine the binding affinity of PK2 for two PK-Rs.	bind
20676	1	6559	5	NULL	NULL	0	NULL	sPLA2-X	NULL	125I-mouse	bind	NULL				PLA2R	NULL	mouse			NULL	COS-7 cells	0	NULL	NULL	NULL	gw60_febslett_478_1_187_s_123	10922494	125I-mouse sPLA2-X binding to mouse PLA2R expressed in COS-7 cells.	bind
24976	1	6559	7	NULL	NULL	NULL	NULL	sPLA2-X 	GP	125I-mouse	binds to					PLA2R	GP	mouse			NULL	COS-7 cells	NULL	NULL	NULL	NULL	gw60_febslett_478_1_187_s_123	10922494	125I-mouse sPLA2-X binding to mouse PLA2R expressed in COS-7 cells.	bind
20677	1	6560	5	NULL	NULL	0	NULL	125I-PDGF-BB	NULL		bind	NULL	specifically			HSC	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_30_28274_s_108	11346654	125I-PDGF-BB binding experiments showed that pretreatment with NAC for 24 h decreased the specific binding of PDGF-BB to HSC (Fig.  1 F).	bind
20678	2	6560	5	NULL	NULL	0	NULL	NAC	NULL	pretreatment with	decrease	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_30_28274_s_108	11346654	125I-PDGF-BB binding experiments showed that pretreatment with NAC for 24 h decreased the specific binding of PDGF-BB to HSC (Fig.  1 F).	bind
24979	1	6560	7	NULL	NULL	NULL	NULL	PDGF-BB	GP	125I	bind		specifically			HSC	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_30_28274_s_108	11346654	125I-PDGF-BB binding experiments showed that pretreatment with NAC for 24 h decreased the specific binding of PDGF-BB to HSC (Fig.  1 F).	bind
24982	2	6560	7	NULL	NULL	NULL	NULL	NAC	Chemical	pretreatment	decrease					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_30_28274_s_108	11346654	125I-PDGF-BB binding experiments showed that pretreatment with NAC for 24 h decreased the specific binding of PDGF-BB to HSC (Fig.  1 F).	bind
20679	1	6561	5	10	NULL	0	NULL	Polymeric IgA		125I	bind					FcalphaR molecules		transfected			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_11_7216_s_262	10066783	125I-Polymeric IgA was bound to transfected FcalphaR molecules and allowed to internalize for various periods in the presence or absence of primaquine.	bind
24986	1	6561	7	NULL	NULL	NULL	NULL	Polymeric IgA	GP	125I	binds					FcalphaR molecules	GP	transfected			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_11_7216_s_262	10066783	125I-Polymeric IgA was bound to transfected FcalphaR molecules and allowed to internalize for various periods in the presence or absence of primaquine.	bind
20680	1	6562	5	NULL	NULL	0	NULL	GalR3 receptor	NULL	rat	is expressed in	NULL				COS-7 cells	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_51_31949_s_8	9405385	125I-Porcine galanin binds the rat GalR3 receptor expressed in COS-7 cells with high affinity ( K d = 0.6 nM) and could be displaced by galanin and galanin fragments and galanin-chimeric peptides.	bind
20681	2	6562	5	NULL	NULL	0	NULL	galanin	NULL	125I-Porcine	bind	NULL	high affinity			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_51_31949_s_8	9405385	125I-Porcine galanin binds the rat GalR3 receptor expressed in COS-7 cells with high affinity ( K d = 0.6 nM) and could be displaced by galanin and galanin fragments and galanin-chimeric peptides.	bind
20682	3	6562	5	10	NULL	0	NULL	galanin			bind					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_31949_s_8	9405385	125I-Porcine galanin binds the rat GalR3 receptor expressed in COS-7 cells with high affinity ( K d = 0.6 nM) and could be displaced by galanin and galanin fragments and galanin-chimeric peptides.	bind
20683	4	6562	5	10	NULL	0	NULL	statement 3			displace					statement 2					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_31949_s_8	9405385	125I-Porcine galanin binds the rat GalR3 receptor expressed in COS-7 cells with high affinity ( K d = 0.6 nM) and could be displaced by galanin and galanin fragments and galanin-chimeric peptides.	bind
20684	5	6562	5	10	NULL	0	NULL	galanin fragments			bind					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_31949_s_8	9405385	125I-Porcine galanin binds the rat GalR3 receptor expressed in COS-7 cells with high affinity ( K d = 0.6 nM) and could be displaced by galanin and galanin fragments and galanin-chimeric peptides.	bind
54423	6	6562	5	10	NULL	0	NULL	statement 5			displace					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_51_31949_s_8	9405385	125I-Porcine galanin binds the rat GalR3 receptor expressed in COS-7 cells with high affinity ( K d = 0.6 nM) and could be displaced by galanin and galanin fragments and galanin-chimeric peptides.	bind
54424	7	6562	5	10	NULL	0	NULL	galanin-chimeric peptides			bind					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_51_31949_s_8	9405385	125I-Porcine galanin binds the rat GalR3 receptor expressed in COS-7 cells with high affinity ( K d = 0.6 nM) and could be displaced by galanin and galanin fragments and galanin-chimeric peptides.	bind
54425	8	6562	5	10	NULL	0	NULL	statement 7			displace					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_51_31949_s_8	9405385	125I-Porcine galanin binds the rat GalR3 receptor expressed in COS-7 cells with high affinity ( K d = 0.6 nM) and could be displaced by galanin and galanin fragments and galanin-chimeric peptides.	bind
24993	2	6562	7	NULL	NULL	NULL	NULL	galanin	GP	125I-Porcine	bind		high affinity			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_31949_s_8	9405385	125I-Porcine galanin binds the rat GalR3 receptor expressed in COS-7 cells with high affinity ( K d = 0.6 nM) and could be displaced by galanin and galanin fragments and galanin-chimeric peptides.	bind
24995	3	6562	7	NULL	NULL	NULL	NULL	galanin	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_31949_s_8	9405385	125I-Porcine galanin binds the rat GalR3 receptor expressed in COS-7 cells with high affinity ( K d = 0.6 nM) and could be displaced by galanin and galanin fragments and galanin-chimeric peptides.	bind
24996	4	6562	7	NULL	NULL	NULL	NULL	galanin fragments	AminoAcid		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_31949_s_8	9405385	125I-Porcine galanin binds the rat GalR3 receptor expressed in COS-7 cells with high affinity ( K d = 0.6 nM) and could be displaced by galanin and galanin fragments and galanin-chimeric peptides.	bind
24998	5	6562	7	NULL	NULL	NULL	NULL	galanin-chimeric peptides	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_31949_s_8	9405385	125I-Porcine galanin binds the rat GalR3 receptor expressed in COS-7 cells with high affinity ( K d = 0.6 nM) and could be displaced by galanin and galanin fragments and galanin-chimeric peptides.	bind
54667	1	6562	7	NULL	NULL	NULL	NULL	GalR3 receptor	GP	rat	expressed in					COS-7 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_31949_s_8	9405385	125I-Porcine galanin binds the rat GalR3 receptor expressed in COS-7 cells with high affinity ( K d = 0.6 nM) and could be displaced by galanin and galanin fragments and galanin-chimeric peptides.	bind
54668	6	6562	7	NULL	NULL	NULL	NULL	statement 3	Process		displace					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_31949_s_8	9405385	125I-Porcine galanin binds the rat GalR3 receptor expressed in COS-7 cells with high affinity ( K d = 0.6 nM) and could be displaced by galanin and galanin fragments and galanin-chimeric peptides.	bind
54669	7	6562	7	NULL	NULL	NULL	NULL	statement 4	Process		displace					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_31949_s_8	9405385	125I-Porcine galanin binds the rat GalR3 receptor expressed in COS-7 cells with high affinity ( K d = 0.6 nM) and could be displaced by galanin and galanin fragments and galanin-chimeric peptides.	bind
54670	8	6562	7	NULL	NULL	NULL	NULL	statement 5	Process		displace					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_51_31949_s_8	9405385	125I-Porcine galanin binds the rat GalR3 receptor expressed in COS-7 cells with high affinity ( K d = 0.6 nM) and could be displaced by galanin and galanin fragments and galanin-chimeric peptides.	bind
20685	1	6563	5	NULL	NULL	0	NULL	CHO cells	NULL		is transfected with	NULL	stably			cDNA	NULL	rabbit 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_44_27217_s_81	8910290	125I-Porcine PYY specifically bound with high affinity ( K d = 50 pM) to membranes from CHO cells stably transfected with the rabbit cDNA.	bind
20686	2	6563	5	10	NULL	0	NULL	PYY		125I-Porcine	bind		specifically;;high affinity			statement 1		membranes from			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27217_s_81	8910290	125I-Porcine PYY specifically bound with high affinity ( K d = 50 pM) to membranes from CHO cells stably transfected with the rabbit cDNA.	bind
25003	1	6563	7	NULL	NULL	NULL	NULL	PYY	GP	125I-Porcine	bind		specifically;;high affinity			membranes	CellComponent	CHO cells			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27217_s_81	8910290	125I-Porcine PYY specifically bound with high affinity ( K d = 50 pM) to membranes from CHO cells stably transfected with the rabbit cDNA.	bind
25006	2	6563	7	NULL	NULL	NULL	NULL	CHO cells	Cell		transfected with		stably			cDNA	NucleicAcid	rabbit			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27217_s_81	8910290	125I-Porcine PYY specifically bound with high affinity ( K d = 50 pM) to membranes from CHO cells stably transfected with the rabbit cDNA.	bind
20687	1	6564	5	10	NULL	0	NULL	PSP-II		125I	bind		lesser extent			polysaccharide zymosan A					NULL		NULL	NULL	NULL	NULL	gw60_febslett_431_2_273_s_63	9708918	125I-PSP-II bound to a lesser extent to the polysaccharide zymosan A, no binding was observed to chondroitin-6-sulfate, and only trace binding to yeast invertase was deteced ( Fig. 1).	bind
20688	2	6564	5	10	NULL	0	NULL	PSP-II		125I	does not bind					chondroitin-6-sulfate					NULL		NULL	NULL	NULL	NULL	gw60_febslett_431_2_273_s_63	9708918	125I-PSP-II bound to a lesser extent to the polysaccharide zymosan A, no binding was observed to chondroitin-6-sulfate, and only trace binding to yeast invertase was deteced ( Fig. 1).	bind
20689	3	6564	5	10	NULL	0	NULL	PSP-II		125I	bind		trace			invertase		yeast			NULL		NULL	NULL	NULL	NULL	gw60_febslett_431_2_273_s_63	9708918	125I-PSP-II bound to a lesser extent to the polysaccharide zymosan A, no binding was observed to chondroitin-6-sulfate, and only trace binding to yeast invertase was deteced ( Fig. 1).	bind
25039	1	6564	7	NULL	NULL	NULL	NULL	PSP-II 	GP	125I	bind		less			zymosan A	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_431_2_273_s_63	9708918	125I-PSP-II bound to a lesser extent to the polysaccharide zymosan A, no binding was observed to chondroitin-6-sulfate, and only trace binding to yeast invertase was deteced ( Fig. 1).	bind
25040	2	6564	7	NULL	NULL	NULL	NULL	PSP-II 	GP	125I	does not bind					chondroitin-6-sulfate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_431_2_273_s_63	9708918	125I-PSP-II bound to a lesser extent to the polysaccharide zymosan A, no binding was observed to chondroitin-6-sulfate, and only trace binding to yeast invertase was deteced ( Fig. 1).	bind
25041	3	6564	7	NULL	NULL	NULL	NULL	PSP-II 	GP	125I	bind		trace			invertase	GP	yeast			NULL		NULL	NULL	NULL	NULL	gw60_febslett_431_2_273_s_63	9708918	125I-PSP-II bound to a lesser extent to the polysaccharide zymosan A, no binding was observed to chondroitin-6-sulfate, and only trace binding to yeast invertase was deteced ( Fig. 1).	bind
67962	4	6564	7	NULL	NULL	0	NULL	zymosan A	Chemical		is a type of					polysaccharide	Chemical				NULL		0	NULL	NULL	NULL	gw60_febslett_431_2_273_s_63	9708918	125I-PSP-II bound to a lesser extent to the polysaccharide zymosan A, no binding was observed to chondroitin-6-sulfate, and only trace binding to yeast invertase was deteced ( Fig. 1).	bind
20690	1	6565	5	10	NULL	0	NULL	TGF-beta		125I	bind					malpha2M					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_40_24982_s_77	8798779	125I-TGF-beta binding to malpha2M was detected by autoradiography.	bind
25042	1	6565	7	NULL	NULL	NULL	NULL	TGF-beta	GP	125I	bind					malpha2M	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_40_24982_s_77	8798779	125I-TGF-beta binding to malpha2M was detected by autoradiography.	bind
20691	1	6566	5	NULL	NULL	0	NULL	125I-TGF-beta1	NULL		bind	NULL	low			TbetaR-II	NULL				NULL	CHO-K1 cells	0	NULL	NULL	NULL	abs-batch0680-0699_j-biol-chem_281_17_16492675_s_5	16492675	125I-TGF-beta1 affinity labeling analysis of cell-surface TGF-beta  receptors reveals that CHO-K1 and CHO-677 cells exhibit low (<1) and high  (>1) ratios of 125I-TGF-beta1 binding to TbetaR-II and TbetaR-I, respectively.	bind
20692	2	6566	5	10	NULL	0	NULL	125I-TGF-beta1	NULL		bind	NULL	low			TbetaR-I	NULL				NULL	CHO-K1 cells	NULL	NULL	NULL	NULL	abs-batch0680-0699_j-biol-chem_281_17_16492675_s_5	16492675	125I-TGF-beta1 affinity labeling analysis of cell-surface TGF-beta  receptors reveals that CHO-K1 and CHO-677 cells exhibit low (<1) and high  (>1) ratios of 125I-TGF-beta1 binding to TbetaR-II and TbetaR-I, respectively.	bind
20693	3	6566	5	10	NULL	0	NULL	125I-TGF-beta1	NULL		bind	NULL	high			TbetaR-II	NULL				NULL	CHO-677 cells	NULL	NULL	NULL	NULL	abs-batch0680-0699_j-biol-chem_281_17_16492675_s_5	16492675	125I-TGF-beta1 affinity labeling analysis of cell-surface TGF-beta  receptors reveals that CHO-K1 and CHO-677 cells exhibit low (<1) and high  (>1) ratios of 125I-TGF-beta1 binding to TbetaR-II and TbetaR-I, respectively.	bind
20694	4	6566	5	NULL	NULL	0	NULL	125I-TGF-beta1	NULL		bind	NULL	high			TbetaR-I	NULL				NULL	CHO-677 cells	NULL	NULL	NULL	NULL	abs-batch0680-0699_j-biol-chem_281_17_16492675_s_5	16492675	125I-TGF-beta1 affinity labeling analysis of cell-surface TGF-beta  receptors reveals that CHO-K1 and CHO-677 cells exhibit low (<1) and high  (>1) ratios of 125I-TGF-beta1 binding to TbetaR-II and TbetaR-I, respectively.	bind
25043	1	6566	7	NULL	NULL	NULL	NULL	125I-TGF-beta1	GP		bind		low			TbetaR-I	GP				NULL	CHO-K1 cells	NULL	NULL	NULL	NULL	abs-batch0680-0699_j-biol-chem_281_17_16492675_s_5	16492675	125I-TGF-beta1 affinity labeling analysis of cell-surface TGF-beta  receptors reveals that CHO-K1 and CHO-677 cells exhibit low (<1) and high  (>1) ratios of 125I-TGF-beta1 binding to TbetaR-II and TbetaR-I, respectively.	bind
25044	2	6566	7	NULL	NULL	NULL	NULL	125I-TGF-beta1	GP		bind		low			TbetaR-II	GP				NULL	CHO-K1 cells	NULL	NULL	NULL	NULL	abs-batch0680-0699_j-biol-chem_281_17_16492675_s_5	16492675	125I-TGF-beta1 affinity labeling analysis of cell-surface TGF-beta  receptors reveals that CHO-K1 and CHO-677 cells exhibit low (<1) and high  (>1) ratios of 125I-TGF-beta1 binding to TbetaR-II and TbetaR-I, respectively.	bind
45757	3	6566	7	NULL	NULL	NULL	NULL	125I-TGF-beta1	GP		bind		high			TbetaR-I	GP				NULL	CHO-677 cells	NULL	NULL	NULL	NULL	abs-batch0680-0699_j-biol-chem_281_17_16492675_s_5	16492675	125I-TGF-beta1 affinity labeling analysis of cell-surface TGF-beta  receptors reveals that CHO-K1 and CHO-677 cells exhibit low (<1) and high  (>1) ratios of 125I-TGF-beta1 binding to TbetaR-II and TbetaR-I, respectively.	bind
45758	4	6566	7	NULL	NULL	NULL	NULL	125I-TGF-beta1	GP		bind		high			TbetaR-II	GP				NULL	CHO-677 cells	NULL	NULL	NULL	NULL	abs-batch0680-0699_j-biol-chem_281_17_16492675_s_5	16492675	125I-TGF-beta1 affinity labeling analysis of cell-surface TGF-beta  receptors reveals that CHO-K1 and CHO-677 cells exhibit low (<1) and high  (>1) ratios of 125I-TGF-beta1 binding to TbetaR-II and TbetaR-I, respectively.	bind
20695	1	6568	5	NULL	NULL	0	NULL	TGF-beta1	NULL	125I	bind	NULL				malpha2M	NULL	purified			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_40_24982_s_150	8798779	125I-TGF-beta1 and 125I-TGF-beta2 bound to purified malpha2M and MUG, as determined by the BS3-rapid cross-linking method.	bind
20696	2	6568	5	NULL	NULL	0	NULL	TGF-beta2	NULL	125I	bind	NULL				malpha2M	NULL	purified			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_40_24982_s_150	8798779	125I-TGF-beta1 and 125I-TGF-beta2 bound to purified malpha2M and MUG, as determined by the BS3-rapid cross-linking method.	bind
20697	3	6568	5	NULL	NULL	0	NULL	TGF-beta1	NULL	125I	bind	NULL				MUG	NULL	purified			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_40_24982_s_150	8798779	125I-TGF-beta1 and 125I-TGF-beta2 bound to purified malpha2M and MUG, as determined by the BS3-rapid cross-linking method.	bind
20698	4	6568	5	NULL	NULL	0	NULL	TGF-beta2	NULL	125I	bind	NULL				MUG	NULL	purified			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_40_24982_s_150	8798779	125I-TGF-beta1 and 125I-TGF-beta2 bound to purified malpha2M and MUG, as determined by the BS3-rapid cross-linking method.	bind
25047	1	6568	7	NULL	NULL	NULL	NULL	TGF-beta1	GP	125I	bind					 malpha2M	GP	purified			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_40_24982_s_150	8798779	125I-TGF-beta1 and 125I-TGF-beta2 bound to purified malpha2M and MUG, as determined by the BS3-rapid cross-linking method.	bind
25048	2	6568	7	NULL	NULL	NULL	NULL	TGF-beta2	GP	125I	bind					malpha2M	GP	purified			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_40_24982_s_150	8798779	125I-TGF-beta1 and 125I-TGF-beta2 bound to purified malpha2M and MUG, as determined by the BS3-rapid cross-linking method.	bind
25049	3	6568	7	NULL	NULL	NULL	NULL	TGF-beta1	GP	125I	bind					MUG	GP	purified			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_40_24982_s_150	8798779	125I-TGF-beta1 and 125I-TGF-beta2 bound to purified malpha2M and MUG, as determined by the BS3-rapid cross-linking method.	bind
25050	4	6568	7	NULL	NULL	NULL	NULL	TGF-beta2	GP	125I	bind					MUG	GP	purified			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_40_24982_s_150	8798779	125I-TGF-beta1 and 125I-TGF-beta2 bound to purified malpha2M and MUG, as determined by the BS3-rapid cross-linking method.	bind
20699	1	6570	5	NULL	NULL	0	NULL	ZIF-1/ Glycodelin-A	NULL	125I	bind	NULL				sperm extracts	NULL	human			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_15_13570_s_248	12571233	125I-ZIF-1/ Glycodelin-A Binding to the Human Sperm Extracts-- Previous study using the same protocol for preparation of human sperm extracts suggested  that the isolated proteins contained mainly membrane proteins ( ).	bind
25052	1	6570	7	NULL	NULL	NULL	NULL	ZIF-1/ Glycodelin-A	GP	125I	bind					Sperm Extracts	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_15_13570_s_248	12571233	125I-ZIF-1/ Glycodelin-A Binding to the Human Sperm Extracts-- Previous study using the same protocol for preparation of human sperm extracts suggested  that the isolated proteins contained mainly membrane proteins ( ).	bind
20700	1	6573	5	NULL	NULL	0	NULL	ZIF-1/ Glycodelin-A	NULL	125I	bind	NULL				sperm extracts	NULL	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_15_13570_s_159	12571233	125I-ZIF-1/ Glycodelin-A Binding to the Human Sperm Extracts-- Sperm extracts was isolated as described ( 25).	bind
25053	1	6573	7	NULL	NULL	NULL	NULL	ZIF-1/ Glycodelin-A	GP	125I	bind					Sperm Extracts	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_15_13570_s_159	12571233	125I-ZIF-1/ Glycodelin-A Binding to the Human Sperm Extracts-- Sperm extracts was isolated as described ( 25).	bind
20701	1	6575	5	NULL	NULL	0	NULL	Sar-1, Ile-8Ang II	NULL	125I	bind	NULL	predominantly			AT1 receptor subtype	NULL				NULL	WT kidneys	NULL	NULL	NULL	NULL	gw60_pnas_100_14_8258_s_75	12829792	125I-[Sar-1,  Ile-8Ang II bound predominantly to the AT1 receptor subtype, in  both WT and  Mas-knockout kidneys  ( Fig. 1  A Center and   C), with low binding to the AT2 receptor  subtype ( Fig. 1  A Right and   C).	bind
20702	2	6575	5	NULL	NULL	0	NULL	Sar-1, Ile-8Ang II	NULL	125I	bind	NULL	predominantly			AT1 receptor subtype	NULL				NULL	Mas-knockout kidneys	NULL	NULL	NULL	NULL	gw60_pnas_100_14_8258_s_75	12829792	125I-[Sar-1,  Ile-8Ang II bound predominantly to the AT1 receptor subtype, in  both WT and  Mas-knockout kidneys  ( Fig. 1  A Center and   C), with low binding to the AT2 receptor  subtype ( Fig. 1  A Right and   C).	bind
20703	3	6575	5	NULL	NULL	0	NULL	Sar-1, Ile-8Ang II	NULL	125I	bind	NULL	low			AT2 receptor subtype	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_14_8258_s_75	12829792	125I-[Sar-1,  Ile-8Ang II bound predominantly to the AT1 receptor subtype, in  both WT and  Mas-knockout kidneys  ( Fig. 1  A Center and   C), with low binding to the AT2 receptor  subtype ( Fig. 1  A Right and   C).	bind
25055	1	6575	7	NULL	NULL	NULL	NULL	Sar-1, Ile-8Ang II	GP	125I	bind		predominantly			AT1 receptor subtype	GP				NULL	WT kidneys	NULL	NULL	NULL	NULL	gw60_pnas_100_14_8258_s_75	12829792	125I-[Sar-1,  Ile-8Ang II bound predominantly to the AT1 receptor subtype, in  both WT and  Mas-knockout kidneys  ( Fig. 1  A Center and   C), with low binding to the AT2 receptor  subtype ( Fig. 1  A Right and   C).	bind
25056	2	6575	7	NULL	NULL	NULL	NULL	Sar-1, Ile-8Ang II	GP	125I	bind		predominantly			AT1 receptor subtype	GP				NULL	Mas-knockout kidneys	NULL	NULL	NULL	NULL	gw60_pnas_100_14_8258_s_75	12829792	125I-[Sar-1,  Ile-8Ang II bound predominantly to the AT1 receptor subtype, in  both WT and  Mas-knockout kidneys  ( Fig. 1  A Center and   C), with low binding to the AT2 receptor  subtype ( Fig. 1  A Right and   C).	bind
25058	3	6575	7	NULL	NULL	NULL	NULL	Sar-1, Ile-8Ang II	GP	125I	bind		low			AT2 receptor subtype	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_14_8258_s_75	12829792	125I-[Sar-1,  Ile-8Ang II bound predominantly to the AT1 receptor subtype, in  both WT and  Mas-knockout kidneys  ( Fig. 1  A Center and   C), with low binding to the AT2 receptor  subtype ( Fig. 1  A Right and   C).	bind
20704	1	6576	5	NULL	NULL	0	NULL	125I-[Tyr3]MP	NULL		bind	NULL				HSR	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_57_6_1235_s_184	10825395	125I-[Tyr3]MP binding to HSR was inhibited by unlabeled [Tyr3]MP (0.1-500 muM) in a concentration-dependent manner at 0 degrees C under the same conditions for 45Ca2+ release experiments (data not shown).	bind
20705	2	6576	5	NULL	NULL	0	NULL	[Tyr3]MP	NULL	unlabeled	inhibit	NULL	concentration dependent			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_57_6_1235_s_184	10825395	125I-[Tyr3]MP binding to HSR was inhibited by unlabeled [Tyr3]MP (0.1-500 muM) in a concentration-dependent manner at 0 degrees C under the same conditions for 45Ca2+ release experiments (data not shown).	bind
25060	1	6576	7	NULL	NULL	NULL	NULL	[Tyr3]MP	Chemical	125I	bind					HSR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_57_6_1235_s_184	10825395	125I-[Tyr3]MP binding to HSR was inhibited by unlabeled [Tyr3]MP (0.1-500 muM) in a concentration-dependent manner at 0 degrees C under the same conditions for 45Ca2+ release experiments (data not shown).	bind
25062	2	6576	7	NULL	NULL	NULL	NULL	[Tyr3]MP	Chemical	unlabeled	inhibits		concentration-dependent			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_57_6_1235_s_184	10825395	125I-[Tyr3]MP binding to HSR was inhibited by unlabeled [Tyr3]MP (0.1-500 muM) in a concentration-dependent manner at 0 degrees C under the same conditions for 45Ca2+ release experiments (data not shown).	bind
20706	1	6577	5	NULL	NULL	0	NULL	[Tyr3]MP	NULL	125I	bind	NULL				HSR	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_57_6_1235_s_182	10825395	125I-[Tyr3]MP Binding to HSR.	bind
25066	1	6577	7	NULL	NULL	NULL	NULL	[Tyr3]MP	Chemical	125I	bind					HSR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_57_6_1235_s_182	10825395	125I-[Tyr3]MP Binding to HSR.	bind
20707	1	6578	5	NULL	NULL	0	NULL	VE-cadherin	NULL		bind	NULL				p120	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_6_743_s_294	16574915	126 - 128   Consequently, the binding of VE-cadherin to p120 and beta-catenin is disrupted, and a rapid internalization and degradation of VE-cadherin occurs via a clathrin-dependent pathway ( Figure 3).	bind
20708	2	6578	5	NULL	NULL	0	NULL	VE-cadherin	NULL		bind	NULL				beta-catenin	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_6_743_s_294	16574915	126 - 128   Consequently, the binding of VE-cadherin to p120 and beta-catenin is disrupted, and a rapid internalization and degradation of VE-cadherin occurs via a clathrin-dependent pathway ( Figure 3).	bind
20743	3	6578	5	NULL	NULL	0	NULL	VE-cadherin	NULL		undergoes	NULL				internalization	NULL	rapid			NULL		0	NULL	NULL	NULL	gw70_circulationres_98_6_743_s_294	16574915	126 - 128   Consequently, the binding of VE-cadherin to p120 and beta-catenin is disrupted, and a rapid internalization and degradation of VE-cadherin occurs via a clathrin-dependent pathway ( Figure 3).	bind
20744	4	6578	5	NULL	NULL	0	NULL	statement 3	NULL		occurs via	NULL				clathrin-dependent pathway	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_6_743_s_294	16574915	126 - 128   Consequently, the binding of VE-cadherin to p120 and beta-catenin is disrupted, and a rapid internalization and degradation of VE-cadherin occurs via a clathrin-dependent pathway ( Figure 3).	bind
20745	5	6578	5	NULL	NULL	0	NULL	VE-cadherin	NULL		undergoes	NULL				degradation	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_6_743_s_294	16574915	126 - 128   Consequently, the binding of VE-cadherin to p120 and beta-catenin is disrupted, and a rapid internalization and degradation of VE-cadherin occurs via a clathrin-dependent pathway ( Figure 3).	bind
20746	6	6578	5	NULL	NULL	0	NULL	statement 5	NULL		occurs via	NULL				clathrin-dependent pathway	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_6_743_s_294	16574915	126 - 128   Consequently, the binding of VE-cadherin to p120 and beta-catenin is disrupted, and a rapid internalization and degradation of VE-cadherin occurs via a clathrin-dependent pathway ( Figure 3).	bind
25067	1	6578	7	NULL	NULL	NULL	NULL	VE-cadherin	GP		binds to					p120	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_743_s_294	16574915	126 - 128   Consequently, the binding of VE-cadherin to p120 and beta-catenin is disrupted, and a rapid internalization and degradation of VE-cadherin occurs via a clathrin-dependent pathway ( Figure 3).	bind
25068	2	6578	7	NULL	NULL	NULL	NULL	VE-cadherin	GP		binds to					beta-catenin	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_743_s_294	16574915	126 - 128   Consequently, the binding of VE-cadherin to p120 and beta-catenin is disrupted, and a rapid internalization and degradation of VE-cadherin occurs via a clathrin-dependent pathway ( Figure 3).	bind
25069	3	6578	7	NULL	NULL	NULL	NULL	statement 1	Process	disruption of	internalizes		rapidly			VE-cadherin	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_743_s_294	16574915	126 - 128   Consequently, the binding of VE-cadherin to p120 and beta-catenin is disrupted, and a rapid internalization and degradation of VE-cadherin occurs via a clathrin-dependent pathway ( Figure 3).	bind
25070	4	6578	7	NULL	NULL	NULL	NULL	VE-cadherin	GP	degradation of	occurs via					clathrin-dependent pathway	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_743_s_294	16574915	126 - 128   Consequently, the binding of VE-cadherin to p120 and beta-catenin is disrupted, and a rapid internalization and degradation of VE-cadherin occurs via a clathrin-dependent pathway ( Figure 3).	bind
25071	5	6578	7	NULL	NULL	NULL	NULL	statement 3	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_743_s_294	16574915	126 - 128   Consequently, the binding of VE-cadherin to p120 and beta-catenin is disrupted, and a rapid internalization and degradation of VE-cadherin occurs via a clathrin-dependent pathway ( Figure 3).	bind
25072	6	6578	7	NULL	NULL	NULL	NULL	statement 2	Process	disruption of	internalizes		rapidly			VE-cadherin	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_743_s_294	16574915	126 - 128   Consequently, the binding of VE-cadherin to p120 and beta-catenin is disrupted, and a rapid internalization and degradation of VE-cadherin occurs via a clathrin-dependent pathway ( Figure 3).	bind
25073	7	6578	7	NULL	NULL	NULL	NULL	statement 6	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_743_s_294	16574915	126 - 128   Consequently, the binding of VE-cadherin to p120 and beta-catenin is disrupted, and a rapid internalization and degradation of VE-cadherin occurs via a clathrin-dependent pathway ( Figure 3).	bind
20747	2	6579	5	NULL	NULL	0	NULL	TZDs	NULL		inhibit	NULL				LPS-inducible genes	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_230_s_160	14592855	126,127  Second, the doses of TZDs that exert maximal inhibitory effects on LPS-inducible genes are significantly higher than their binding affinity to PPARgamma.	bind
20748	1	6579	5	NULL	NULL	0	NULL	LPS-inducible genes	NULL		bind	NULL				PPARgamma	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_230_s_160	14592855	126,127  Second, the doses of TZDs that exert maximal inhibitory effects on LPS-inducible genes are significantly higher than their binding affinity to PPARgamma.	bind
30305	3	6579	5	NULL	NULL	0	NULL	statement 2	NULL		is higher than	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_230_s_160	14592855	126,127  Second, the doses of TZDs that exert maximal inhibitory effects on LPS-inducible genes are significantly higher than their binding affinity to PPARgamma.	bind
25075	1	6579	7	NULL	NULL	NULL	NULL	LPS-inducible genes	GP		bind					PPARgamma	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_230_s_160	14592855	126,127  Second, the doses of TZDs that exert maximal inhibitory effects on LPS-inducible genes are significantly higher than their binding affinity to PPARgamma.	bind
25077	2	6579	7	NULL	NULL	NULL	NULL	TZDs	Chemical		inhibits					LPS-inducible genes	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_230_s_160	14592855	126,127  Second, the doses of TZDs that exert maximal inhibitory effects on LPS-inducible genes are significantly higher than their binding affinity to PPARgamma.	bind
25078	3	6579	7	NULL	NULL	NULL	NULL	statement 2	Process		is higher than					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_230_s_160	14592855	126,127  Second, the doses of TZDs that exert maximal inhibitory effects on LPS-inducible genes are significantly higher than their binding affinity to PPARgamma.	bind
20749	1	6580	5	NULL	NULL	0	NULL	12CO	NULL		bind	NULL				Ch-CooA	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_5_3269_s_115	15537640	12CO-bound Ch-CooA ( a), 13CO-bound Ch-CooA ( b), and the difference spectrum ( a -  b) ( c).	bind
20750	2	6580	5	NULL	NULL	0	NULL	13CO	NULL		bind	NULL				Ch-CooA	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_5_3269_s_115	15537640	12CO-bound Ch-CooA ( a), 13CO-bound Ch-CooA ( b), and the difference spectrum ( a -  b) ( c).	bind
25080	1	6580	7	NULL	NULL	NULL	NULL	12CO	Chemical		bind					Ch-CooA	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_5_3269_s_115	15537640	12CO-bound Ch-CooA ( a), 13CO-bound Ch-CooA ( b), and the difference spectrum ( a -  b) ( c).	bind
25081	2	6580	7	NULL	NULL	NULL	NULL	13CO	Chemical		bind					Ch-CooA	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_5_3269_s_115	15537640	12CO-bound Ch-CooA ( a), 13CO-bound Ch-CooA ( b), and the difference spectrum ( a -  b) ( c).	bind
20751	1	6581	5	NULL	NULL	0	NULL	SDF-1	NULL		mediate	NULL				chemotactic responses	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_139_3_651_s_250	9348282	12G5 can partially inhibit SDF-1-mediated chemotactic responses, SDF-1-induced modulation of intracellular  calcium, and SDF-1 binding to CXCR4 ( 8,  30).	bind
20752	2	6581	5	NULL	NULL	0	NULL	12G5	NULL		inhibit	NULL	partially			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_139_3_651_s_250	9348282	12G5 can partially inhibit SDF-1-mediated chemotactic responses, SDF-1-induced modulation of intracellular  calcium, and SDF-1 binding to CXCR4 ( 8,  30).	bind
20753	3	6581	5	NULL	NULL	0	NULL	SDF-1	NULL		induces	NULL				intracellular calcium	NULL	modulation of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_139_3_651_s_250	9348282	12G5 can partially inhibit SDF-1-mediated chemotactic responses, SDF-1-induced modulation of intracellular  calcium, and SDF-1 binding to CXCR4 ( 8,  30).	bind
20754	4	6581	5	NULL	NULL	0	NULL	12G5	NULL		inhibit	NULL	partially			statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_139_3_651_s_250	9348282	12G5 can partially inhibit SDF-1-mediated chemotactic responses, SDF-1-induced modulation of intracellular  calcium, and SDF-1 binding to CXCR4 ( 8,  30).	bind
20755	5	6581	5	NULL	NULL	0	NULL	SDF-1	NULL		bind	NULL				CXCR4	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_139_3_651_s_250	9348282	12G5 can partially inhibit SDF-1-mediated chemotactic responses, SDF-1-induced modulation of intracellular  calcium, and SDF-1 binding to CXCR4 ( 8,  30).	bind
20756	6	6581	5	NULL	NULL	0	NULL	12G5	NULL		inhibit	NULL	partially			statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_139_3_651_s_250	9348282	12G5 can partially inhibit SDF-1-mediated chemotactic responses, SDF-1-induced modulation of intracellular  calcium, and SDF-1 binding to CXCR4 ( 8,  30).	bind
25092	1	6581	7	NULL	NULL	NULL	NULL	SDF-1	GP		mediates					chemotactic responses	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_139_3_651_s_250	9348282	12G5 can partially inhibit SDF-1-mediated chemotactic responses, SDF-1-induced modulation of intracellular  calcium, and SDF-1 binding to CXCR4 ( 8,  30).	bind
25093	2	6581	7	NULL	NULL	NULL	NULL	12G5	GP		inhibit		partially			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_139_3_651_s_250	9348282	12G5 can partially inhibit SDF-1-mediated chemotactic responses, SDF-1-induced modulation of intracellular  calcium, and SDF-1 binding to CXCR4 ( 8,  30).	bind
25094	3	6581	7	NULL	NULL	NULL	NULL	SDF-1	GP		induce					 calcium	Chemical	modulation of;; intracellular			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_139_3_651_s_250	9348282	12G5 can partially inhibit SDF-1-mediated chemotactic responses, SDF-1-induced modulation of intracellular  calcium, and SDF-1 binding to CXCR4 ( 8,  30).	bind
25095	4	6581	7	NULL	NULL	NULL	NULL	SDF-1	GP		bind					CXCR4	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_139_3_651_s_250	9348282	12G5 can partially inhibit SDF-1-mediated chemotactic responses, SDF-1-induced modulation of intracellular  calcium, and SDF-1 binding to CXCR4 ( 8,  30).	bind
31407	5	6581	7	NULL	NULL	NULL	NULL	12G5	GP		inhibit		partially			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_139_3_651_s_250	9348282	12G5 can partially inhibit SDF-1-mediated chemotactic responses, SDF-1-induced modulation of intracellular  calcium, and SDF-1 binding to CXCR4 ( 8,  30).	bind
31408	6	6581	7	NULL	NULL	NULL	NULL	12G5	GP		inhibit		partially			statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_139_3_651_s_250	9348282	12G5 can partially inhibit SDF-1-mediated chemotactic responses, SDF-1-induced modulation of intracellular  calcium, and SDF-1 binding to CXCR4 ( 8,  30).	bind
20759	1	6582	5	NULL	NULL	0	NULL	1D4	NULL		bind	NULL				CXCR4-C9	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_5_3378_s_148	12433920	12G5 only recognizes conformationally intact CXCR4, whereas the 1D4 can bind all CXCR4-C9, regardless of conformation.	bind
20760	2	6582	5	NULL	NULL	0	NULL	12G5	NULL		recognizes	NULL				CXCR4	NULL	conformationally intact			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_5_3378_s_148	12433920	12G5 only recognizes conformationally intact CXCR4, whereas the 1D4 can bind all CXCR4-C9, regardless of conformation.	bind
30306	3	6582	5	NULL	NULL	0	NULL	statement 2	NULL		is regardless of	NULL				conformation	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_5_3378_s_148	12433920	12G5 only recognizes conformationally intact CXCR4, whereas the 1D4 can bind all CXCR4-C9, regardless of conformation.	bind
25096	1	6582	7	NULL	NULL	NULL	NULL	12G5	GP		recognizes					CXCR4	GP	conformationally intact			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_5_3378_s_148	12433920	12G5 only recognizes conformationally intact CXCR4, whereas the 1D4 can bind all CXCR4-C9, regardless of conformation.	bind
25097	2	6582	7	NULL	NULL	NULL	NULL	1D4	GP		bind					 CXCR4-C9	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_5_3378_s_148	12433920	12G5 only recognizes conformationally intact CXCR4, whereas the 1D4 can bind all CXCR4-C9, regardless of conformation.	bind
25098	3	6582	7	NULL	NULL	NULL	NULL	statement 2	Process		is regardless of					conformation	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_5_3378_s_148	12433920	12G5 only recognizes conformationally intact CXCR4, whereas the 1D4 can bind all CXCR4-C9, regardless of conformation.	bind
20761	1	6583	5	NULL	NULL	0	NULL	TFIIB	NULL		bind	NULL				p300	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_171	10330164	12S E1A inhibits the binding of TFIIB to p300, while 13S E1A has no effect on the p300-TFIIB interaction.	bind
20762	2	6583	5	NULL	NULL	0	NULL	12S E1A	NULL		inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_171	10330164	12S E1A inhibits the binding of TFIIB to p300, while 13S E1A has no effect on the p300-TFIIB interaction.	bind
20763	3	6583	5	NULL	NULL	0	NULL	13S E1A	NULL		does not effect	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_171	10330164	12S E1A inhibits the binding of TFIIB to p300, while 13S E1A has no effect on the p300-TFIIB interaction.	bind
25099	1	6583	7	NULL	NULL	NULL	NULL	TFIIB	GP		bind					p300	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_171	10330164	12S E1A inhibits the binding of TFIIB to p300, while 13S E1A has no effect on the p300-TFIIB interaction.	bind
25100	2	6583	7	NULL	NULL	NULL	NULL	12S E1A	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_171	10330164	12S E1A inhibits the binding of TFIIB to p300, while 13S E1A has no effect on the p300-TFIIB interaction.	bind
25101	3	6583	7	NULL	NULL	NULL	NULL	13S E1A	GP		has no effect on					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_171	10330164	12S E1A inhibits the binding of TFIIB to p300, while 13S E1A has no effect on the p300-TFIIB interaction.	bind
20764	1	6584	5	NULL	NULL	0	NULL	DNA ligase IV	NULL		bind	NULL		motif located between BRCT domains		XRCC4	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_23_4642_s_270	11095673	13       Grawunder,U., Zimmer,D. and Leiber,M.R. (1998) DNA ligase IV binds to XRCC4 via a motif located between rather than within its BRCT domains.	bind
25102	1	6584	7	NULL	NULL	NULL	NULL	DNA ligase IV	GP		binds to			motif between BRCT domain		XRCC4	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_23_4642_s_270	11095673	13       Grawunder,U., Zimmer,D. and Leiber,M.R. (1998) DNA ligase IV binds to XRCC4 via a motif located between rather than within its BRCT domains.	bind
20765	1	6585	5	NULL	NULL	0	NULL	H19 RNA	NULL		bind	NULL				IGF-II mRNA-binding protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_1_189_s_210	11125087	13       Runge,S., Nielsen,F.C., Nielsen,J., Lykke-Andersen,J., Wewer,U.M. and Christiansen,J. (2000) H19 RNA binds four molecules of IGF-II mRNA-binding protein.	bind
25103	1	6585	7	NULL	NULL	NULL	NULL	H19 RNA	NucleicAcid		binds					IGF-II mRNA-binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_1_189_s_210	11125087	13       Runge,S., Nielsen,F.C., Nielsen,J., Lykke-Andersen,J., Wewer,U.M. and Christiansen,J. (2000) H19 RNA binds four molecules of IGF-II mRNA-binding protein.	bind
20766	1	6586	5	NULL	NULL	0	NULL	CNP	NULL		bind	NULL				NPR-B	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_96_7_2272_s_25	9337200	13  CNP binds to NPR-B, which contains guanylyl cyclase 14  and induces the production of cGMP.	bind
20767	2	6586	5	10	NULL	0	NULL	NPR-B			contains					guanylyl cyclase					NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_7_2272_s_25	9337200	13  CNP binds to NPR-B, which contains guanylyl cyclase 14  and induces the production of cGMP.	bind
20768	3	6586	5	NULL	NULL	0	NULL	NPR-B	NULL		induces	NULL				cGMP	NULL	production of			NULL		0	NULL	NULL	NULL	gw60_circulation_96_7_2272_s_25	9337200	13  CNP binds to NPR-B, which contains guanylyl cyclase 14  and induces the production of cGMP.	bind
25104	1	6586	7	NULL	NULL	NULL	NULL	CNP	GP		binds to					NPR-B	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_7_2272_s_25	9337200	13  CNP binds to NPR-B, which contains guanylyl cyclase 14  and induces the production of cGMP.	bind
25105	2	6586	7	NULL	NULL	NULL	NULL	NPR-B	GP		contains					guanylyl cyclase	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_7_2272_s_25	9337200	13  CNP binds to NPR-B, which contains guanylyl cyclase 14  and induces the production of cGMP.	bind
25106	3	6586	7	NULL	NULL	NULL	NULL	statement 1	Process		induces					cGMP	Chemical	production of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_7_2272_s_25	9337200	13  CNP binds to NPR-B, which contains guanylyl cyclase 14  and induces the production of cGMP.	bind
20769	1	6587	5	NULL	NULL	0	NULL	 CT-1	NULL		bind	NULL				gp130-LIF receptor complex	NULL				NULL	in myocytes	0	NULL	NULL	NULL	gw60_circulationres_88_7_727_s_23	11304496	13  CT-1 binds to the gp130-LIF receptor complex in myocytes, activating the JAK-STAT pathway and inducing hypertrophic responses.	bind
20770	2	6587	5	NULL	NULL	0	NULL	statement 1	NULL		activates	NULL				JAK-STAT pathway	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_88_7_727_s_23	11304496	13  CT-1 binds to the gp130-LIF receptor complex in myocytes, activating the JAK-STAT pathway and inducing hypertrophic responses.	bind
20771	3	6587	5	NULL	NULL	0	NULL	statement 1	NULL		induces	NULL				hypertrophic responses	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_88_7_727_s_23	11304496	13  CT-1 binds to the gp130-LIF receptor complex in myocytes, activating the JAK-STAT pathway and inducing hypertrophic responses.	bind
25107	1	6587	7	NULL	NULL	NULL	NULL	CT-1	GP		binds to					gp130-LIF receptor complex	GP				NULL	myocytes	NULL	NULL	NULL	NULL	gw60_circulationres_88_7_727_s_23	11304496	13  CT-1 binds to the gp130-LIF receptor complex in myocytes, activating the JAK-STAT pathway and inducing hypertrophic responses.	bind
25108	2	6587	7	NULL	NULL	NULL	NULL	statement 1	Process		activates					JAK-STAT pathway	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_7_727_s_23	11304496	13  CT-1 binds to the gp130-LIF receptor complex in myocytes, activating the JAK-STAT pathway and inducing hypertrophic responses.	bind
25109	3	6587	7	NULL	NULL	NULL	NULL	statement 1	Process		induce					hypertrophic responses	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_7_727_s_23	11304496	13  CT-1 binds to the gp130-LIF receptor complex in myocytes, activating the JAK-STAT pathway and inducing hypertrophic responses.	bind
20792	1	6588	5	NULL	NULL	0	NULL	FHC LDL	NULL		binding	NULL	defective			LDL receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_137_s_31	8548414	13  In addition, the FHC LDL shows defective binding to the LDL receptor 21  and delayed plasma clearance 22  that seemed to be independent of the LDL receptor.	bind
20795	2	6588	5	NULL	NULL	0	NULL	FHC LDL	NULL		shows	NULL				plasma clearance	NULL	delayed			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_137_s_31	8548414	13  In addition, the FHC LDL shows defective binding to the LDL receptor 21  and delayed plasma clearance 22  that seemed to be independent of the LDL receptor.	bind
20796	3	6588	5	NULL	NULL	0	NULL	plasma clearance	NULL		is independent of	NULL				LDL receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_137_s_31	8548414	13  In addition, the FHC LDL shows defective binding to the LDL receptor 21  and delayed plasma clearance 22  that seemed to be independent of the LDL receptor.	bind
25110	1	6588	7	NULL	NULL	NULL	NULL	FHC LDL	GP		bind		defective			LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_137_s_31	8548414	13  In addition, the FHC LDL shows defective binding to the LDL receptor 21  and delayed plasma clearance 22  that seemed to be independent of the LDL receptor.	bind
25111	2	6588	7	NULL	NULL	NULL	NULL	FHC LDL	GP		shows					plasma clearance	Process	delayed			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_137_s_31	8548414	13  In addition, the FHC LDL shows defective binding to the LDL receptor 21  and delayed plasma clearance 22  that seemed to be independent of the LDL receptor.	bind
25112	3	6588	7	NULL	NULL	NULL	NULL	statement 2	Process		is independent of					LDL receptor	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_137_s_31	8548414	13  In addition, the FHC LDL shows defective binding to the LDL receptor 21  and delayed plasma clearance 22  that seemed to be independent of the LDL receptor.	bind
20783	1	6589	5	NULL	NULL	0	NULL	 NF-kappaB	NULL		is present as	NULL				heterodimer	NULL				NULL	in cytosol	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1116_s_199	10764682	13  NF-kappaB is present in cytosol as a heterodimer composed of NF-kappaB1 (P50) and Rel (P65) subunits bound to an inhibitor protein, I-kappaB.	bind
20785	2	6589	5	NULL	NULL	0	NULL	NF-kappaB	NULL		is composed of	NULL					NULL		P50 subunit		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1116_s_199	10764682	13  NF-kappaB is present in cytosol as a heterodimer composed of NF-kappaB1 (P50) and Rel (P65) subunits bound to an inhibitor protein, I-kappaB.	bind
20786	3	6589	5	10	NULL	0	NULL	p50 subunit			is					NF-kappaB1					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1116_s_199	10764682	13  NF-kappaB is present in cytosol as a heterodimer composed of NF-kappaB1 (P50) and Rel (P65) subunits bound to an inhibitor protein, I-kappaB.	bind
20788	4	6589	5	NULL	NULL	0	NULL	NF-kappaB	NULL		is composed of	NULL					NULL		p65 subunit		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1116_s_199	10764682	13  NF-kappaB is present in cytosol as a heterodimer composed of NF-kappaB1 (P50) and Rel (P65) subunits bound to an inhibitor protein, I-kappaB.	bind
20790	5	6589	5	10	NULL	0	NULL	p65 subunit			is					Rel					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1116_s_199	10764682	13  NF-kappaB is present in cytosol as a heterodimer composed of NF-kappaB1 (P50) and Rel (P65) subunits bound to an inhibitor protein, I-kappaB.	bind
20791	6	6589	5	NULL	NULL	0	NULL	NF-kappaB	NULL		bind	NULL				I-kappaB protein	NULL				NULL	in cytosol	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1116_s_199	10764682	13  NF-kappaB is present in cytosol as a heterodimer composed of NF-kappaB1 (P50) and Rel (P65) subunits bound to an inhibitor protein, I-kappaB.	bind
30307	7	6589	5	NULL	NULL	0	NULL	NF-kappa-B	NULL		is a type of	NULL				heterodimer	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1116_s_199	10764682	13  NF-kappaB is present in cytosol as a heterodimer composed of NF-kappaB1 (P50) and Rel (P65) subunits bound to an inhibitor protein, I-kappaB.	bind
30308	8	6589	5	NULL	NULL	0	NULL	I-kappaB	NULL		is a type of	NULL				inhibitor protein	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1116_s_199	10764682	13  NF-kappaB is present in cytosol as a heterodimer composed of NF-kappaB1 (P50) and Rel (P65) subunits bound to an inhibitor protein, I-kappaB.	bind
54453	9	6589	5	10	NULL	0	NULL	statement 2			occurs along with					statement 4					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1116_s_199	10764682	13  NF-kappaB is present in cytosol as a heterodimer composed of NF-kappaB1 (P50) and Rel (P65) subunits bound to an inhibitor protein, I-kappaB.	bind
25113	1	6589	7	NULL	NULL	NULL	NULL	NF-kappaB 	GP		is present in					cytosol	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1116_s_199	10764682	13  NF-kappaB is present in cytosol as a heterodimer composed of NF-kappaB1 (P50) and Rel (P65) subunits bound to an inhibitor protein, I-kappaB.	bind
25114	2	6589	7	NULL	NULL	NULL	NULL	NF-kappaB	GP		is composed of								P50 subunit		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1116_s_199	10764682	13  NF-kappaB is present in cytosol as a heterodimer composed of NF-kappaB1 (P50) and Rel (P65) subunits bound to an inhibitor protein, I-kappaB.	bind
25115	3	6589	7	NULL	NULL	NULL	NULL	NF-kappaB	GP		is composed of								P65 subunit		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1116_s_199	10764682	13  NF-kappaB is present in cytosol as a heterodimer composed of NF-kappaB1 (P50) and Rel (P65) subunits bound to an inhibitor protein, I-kappaB.	bind
25116	4	6589	7	NULL	NULL	NULL	NULL	NF-kappaB	GP		bind					 I-kappaB	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1116_s_199	10764682	13  NF-kappaB is present in cytosol as a heterodimer composed of NF-kappaB1 (P50) and Rel (P65) subunits bound to an inhibitor protein, I-kappaB.	bind
25117	5	6589	7	NULL	NULL	NULL	NULL	P50 subunit	GP		is					NF-kappaB1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1116_s_199	10764682	13  NF-kappaB is present in cytosol as a heterodimer composed of NF-kappaB1 (P50) and Rel (P65) subunits bound to an inhibitor protein, I-kappaB.	bind
25118	6	6589	7	NULL	NULL	NULL	NULL	P65 subunit	GP 		is					Rel	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1116_s_199	10764682	13  NF-kappaB is present in cytosol as a heterodimer composed of NF-kappaB1 (P50) and Rel (P65) subunits bound to an inhibitor protein, I-kappaB.	bind
32057	7	6589	7	NULL	NULL	NULL	NULL	NF-kappaB	GP		is a type of					heterodimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1116_s_199	10764682	13  NF-kappaB is present in cytosol as a heterodimer composed of NF-kappaB1 (P50) and Rel (P65) subunits bound to an inhibitor protein, I-kappaB.	bind
32058	8	6589	7	NULL	NULL	NULL	NULL	I-kappaB	GP		is a type of					inhibitor protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1116_s_199	10764682	13  NF-kappaB is present in cytosol as a heterodimer composed of NF-kappaB1 (P50) and Rel (P65) subunits bound to an inhibitor protein, I-kappaB.	bind
54454	9	6589	7	NULL	NULL	NULL	NULL	statement 2	Process		occurs along with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1116_s_199	10764682	13  NF-kappaB is present in cytosol as a heterodimer composed of NF-kappaB1 (P50) and Rel (P65) subunits bound to an inhibitor protein, I-kappaB.	bind
20779	1	6590	5	NULL	NULL	0	NULL	TRADD	NULL		bind	NULL		C-terminal portion		FADD	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_3_997_s_27	10702415	13  The C-terminal portion of TRADD binds the death domain-containing protein FADD, resulting in apoptosis.	bind
20781	2	6590	5	NULL	NULL	0	NULL	statement 1	NULL		results in	NULL				apoptosis	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_3_997_s_27	10702415	13  The C-terminal portion of TRADD binds the death domain-containing protein FADD, resulting in apoptosis.	bind
30309	3	6590	5	NULL	NULL	0	NULL	FADD	NULL		is a type of	NULL				death domain-containing protein	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_3_997_s_27	10702415	13  The C-terminal portion of TRADD binds the death domain-containing protein FADD, resulting in apoptosis.	bind
25119	1	6590	7	NULL	NULL	NULL	NULL	TRADD	GP		binds			C-terminal		FADD	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_3_997_s_27	10702415	13  The C-terminal portion of TRADD binds the death domain-containing protein FADD, resulting in apoptosis.	bind
25120	2	6590	7	NULL	NULL	NULL	NULL	statement 1	Process		results in					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_3_997_s_27	10702415	13  The C-terminal portion of TRADD binds the death domain-containing protein FADD, resulting in apoptosis.	bind
31441	3	6590	7	NULL	NULL	NULL	NULL	FADD	GP		is a type of					death domain-containing protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_3_997_s_27	10702415	13  The C-terminal portion of TRADD binds the death domain-containing protein FADD, resulting in apoptosis.	bind
20773	1	6591	5	NULL	NULL	0	NULL	decorin	NULL		bind	NULL				collagen	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_4_847_s_155	10195908	13  These experiments showed that when decorin was first allowed to bind to the collagen, binding of LDL to the decorin-collagen complex was >10 fold greaterR than to collagen alone.	bind
20774	2	6591	5	NULL	NULL	0	NULL	LDL	NULL		bind	NULL				decorin-collagen complex	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_4_847_s_155	10195908	13  These experiments showed that when decorin was first allowed to bind to the collagen, binding of LDL to the decorin-collagen complex was >10 fold greaterR than to collagen alone.	bind
20775	3	6591	5	10	NULL	0	NULL	LDL	NULL		bind	NULL				collagen	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_4_847_s_155	10195908	13  These experiments showed that when decorin was first allowed to bind to the collagen, binding of LDL to the decorin-collagen complex was >10 fold greaterR than to collagen alone.	bind
20776	4	6591	5	NULL	NULL	0	NULL	statement 2	NULL		greater than	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_4_847_s_155	10195908	13  These experiments showed that when decorin was first allowed to bind to the collagen, binding of LDL to the decorin-collagen complex was >10 fold greaterR than to collagen alone.	bind
20777	5	6591	5	NULL	NULL	0	NULL	statement 1	NULL		is required for	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_4_847_s_155	10195908	13  These experiments showed that when decorin was first allowed to bind to the collagen, binding of LDL to the decorin-collagen complex was >10 fold greaterR than to collagen alone.	bind
25121	1	6591	7	NULL	NULL	NULL	NULL	decorin 	GP		bind					collagen	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_4_847_s_155	10195908	13  These experiments showed that when decorin was first allowed to bind to the collagen, binding of LDL to the decorin-collagen complex was >10 fold greaterR than to collagen alone.	bind
25122	2	6591	7	NULL	NULL	NULL	NULL	LDL	GP		bind					decorin-collagen complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_4_847_s_155	10195908	13  These experiments showed that when decorin was first allowed to bind to the collagen, binding of LDL to the decorin-collagen complex was >10 fold greaterR than to collagen alone.	bind
25123	3	6591	7	NULL	NULL	NULL	NULL	LDL	GP		bind					collagen	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_4_847_s_155	10195908	13  These experiments showed that when decorin was first allowed to bind to the collagen, binding of LDL to the decorin-collagen complex was >10 fold greaterR than to collagen alone.	bind
25124	4	6591	7	NULL	NULL	NULL	NULL	statement 2	Process		is greater than					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_4_847_s_155	10195908	13  These experiments showed that when decorin was first allowed to bind to the collagen, binding of LDL to the decorin-collagen complex was >10 fold greaterR than to collagen alone.	bind
20772	1	6592	5	10	NULL	0	NULL	thrombin			bind					hirudin-CD4					NULL		NULL	NULL	NULL	NULL	gw60_circulation_98_24_2744_s_102	9851962	13  Thrombin binding to the hirudin-CD4 fusion protein was assessed after preincubation of the enzyme with either native hirudin, the tripeptide active site inhibitor PPACK, or a synthetic COOH-terminal hirudin dodecapeptide.	bind
54455	2	6592	5	10	NULL	0	NULL	hirudin-CD4			is a type of					fusion protein					NULL		0	NULL	NULL	NULL	gw60_circulation_98_24_2744_s_102	9851962	13  Thrombin binding to the hirudin-CD4 fusion protein was assessed after preincubation of the enzyme with either native hirudin, the tripeptide active site inhibitor PPACK, or a synthetic COOH-terminal hirudin dodecapeptide.	bind
25125	1	6592	7	NULL	NULL	NULL	NULL	Thrombin	GP		binds					hirudin-CD4	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_98_24_2744_s_102	9851962	13  Thrombin binding to the hirudin-CD4 fusion protein was assessed after preincubation of the enzyme with either native hirudin, the tripeptide active site inhibitor PPACK, or a synthetic COOH-terminal hirudin dodecapeptide.	bind
54456	2	6592	7	NULL	NULL	NULL	NULL	hirudin-CD4	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_98_24_2744_s_102	9851962	13  Thrombin binding to the hirudin-CD4 fusion protein was assessed after preincubation of the enzyme with either native hirudin, the tripeptide active site inhibitor PPACK, or a synthetic COOH-terminal hirudin dodecapeptide.	bind
20799	1	6593	5	NULL	NULL	0	NULL	TGF ligand	NULL		bind	NULL				type II receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_28	10934147	13  Type III receptor (also known as betaglycan) is a membrane-anchored proteoglycan that facilitates TGF ligand binding to the type II receptor.	bind
20800	2	6593	5	10	NULL	0	NULL	Type III receptor			is a synonym of					betaglycan					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_28	10934147	13  Type III receptor (also known as betaglycan) is a membrane-anchored proteoglycan that facilitates TGF ligand binding to the type II receptor.	bind
20801	3	6593	5	10	NULL	0	NULL	Type III receptor			facilitates					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_28	10934147	13  Type III receptor (also known as betaglycan) is a membrane-anchored proteoglycan that facilitates TGF ligand binding to the type II receptor.	bind
54457	4	6593	5	10	NULL	0	NULL	Type III receptor			is a type of					membrane-anchored proteoglycan					NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_28	10934147	13  Type III receptor (also known as betaglycan) is a membrane-anchored proteoglycan that facilitates TGF ligand binding to the type II receptor.	bind
25126	1	6593	7	NULL	NULL	NULL	NULL	 TGF ligand	GP		bind					type II receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_28	10934147	13  Type III receptor (also known as betaglycan) is a membrane-anchored proteoglycan that facilitates TGF ligand binding to the type II receptor.	bind
25127	2	6593	7	NULL	NULL	NULL	NULL	Type III receptor	GP		facilitates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_28	10934147	13  Type III receptor (also known as betaglycan) is a membrane-anchored proteoglycan that facilitates TGF ligand binding to the type II receptor.	bind
25128	3	6593	7	NULL	NULL	NULL	NULL	Type III receptor	GP		is 					betaglycan	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_28	10934147	13  Type III receptor (also known as betaglycan) is a membrane-anchored proteoglycan that facilitates TGF ligand binding to the type II receptor.	bind
54458	4	6593	7	NULL	NULL	NULL	NULL	Type III receptor	GP		is a type of					membrane-anchored proteoglycan	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_28	10934147	13  Type III receptor (also known as betaglycan) is a membrane-anchored proteoglycan that facilitates TGF ligand binding to the type II receptor.	bind
20805	1	6594	5	NULL	NULL	0	NULL	VEGF	NULL		bind	NULL				Flk-1	NULL				NULL	in endothelial cells	NULL	NULL	NULL	NULL	gw60_circulationres_85_2_192_s_36	10417401	13  VEGF binding to receptor tyrosinekinase  Flk-1 and Flt-1 14  expressed in endothelial cells is required for normal vascularization.	bind
20806	2	6594	5	NULL	NULL	0	NULL	VEGF	NULL		bind	NULL				Flt-1	NULL				NULL	in endothelial cells	NULL	NULL	NULL	NULL	gw60_circulationres_85_2_192_s_36	10417401	13  VEGF binding to receptor tyrosinekinase  Flk-1 and Flt-1 14  expressed in endothelial cells is required for normal vascularization.	bind
20807	3	6594	5	NULL	NULL	0	NULL	statement 1	NULL		is required for	NULL				normal vascularization	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_2_192_s_36	10417401	13  VEGF binding to receptor tyrosinekinase  Flk-1 and Flt-1 14  expressed in endothelial cells is required for normal vascularization.	bind
20809	4	6594	5	NULL	NULL	0	NULL	statement 2	NULL		is required for	NULL				normal vascularization	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_2_192_s_36	10417401	13  VEGF binding to receptor tyrosinekinase  Flk-1 and Flt-1 14  expressed in endothelial cells is required for normal vascularization.	bind
54459	5	6594	5	10	NULL	0	NULL	Flk-1			is a type of					receptor tyrosinekinase					NULL		0	NULL	NULL	NULL	gw60_circulationres_85_2_192_s_36	10417401	13  VEGF binding to receptor tyrosinekinase  Flk-1 and Flt-1 14  expressed in endothelial cells is required for normal vascularization.	bind
54460	6	6594	5	10	NULL	0	NULL	Flt-1			is a type of					receptor tyrosinekinase					NULL		0	NULL	NULL	NULL	gw60_circulationres_85_2_192_s_36	10417401	13  VEGF binding to receptor tyrosinekinase  Flk-1 and Flt-1 14  expressed in endothelial cells is required for normal vascularization.	bind
25129	1	6594	7	NULL	NULL	NULL	NULL	VEGF	GP		binds to					 Flk-1	GP				NULL	endothelial cells	NULL	NULL	NULL	NULL	gw60_circulationres_85_2_192_s_36	10417401	13  VEGF binding to receptor tyrosinekinase  Flk-1 and Flt-1 14  expressed in endothelial cells is required for normal vascularization.	bind
25130	2	6594	7	NULL	NULL	NULL	NULL	VEGF	GP		binds to					 Flt-1	GP				NULL	endothelial cells	NULL	NULL	NULL	NULL	gw60_circulationres_85_2_192_s_36	10417401	13  VEGF binding to receptor tyrosinekinase  Flk-1 and Flt-1 14  expressed in endothelial cells is required for normal vascularization.	bind
25131	3	6594	7	NULL	NULL	NULL	NULL	statement 1	Process		is required for					normal vascularization	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_2_192_s_36	10417401	13  VEGF binding to receptor tyrosinekinase  Flk-1 and Flt-1 14  expressed in endothelial cells is required for normal vascularization.	bind
25132	4	6594	7	NULL	NULL	NULL	NULL	statement 2	Process		is required for					normal vascularization	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_2_192_s_36	10417401	13  VEGF binding to receptor tyrosinekinase  Flk-1 and Flt-1 14  expressed in endothelial cells is required for normal vascularization.	bind
31442	5	6594	7	NULL	NULL	NULL	NULL	 Flk-1	GP		is a type of					receptor tyrosinekinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_2_192_s_36	10417401	13  VEGF binding to receptor tyrosinekinase  Flk-1 and Flt-1 14  expressed in endothelial cells is required for normal vascularization.	bind
31443	6	6594	7	NULL	NULL	NULL	NULL	Flt-1	GP		is a type of					receptor tyrosine kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_2_192_s_36	10417401	13  VEGF binding to receptor tyrosinekinase  Flk-1 and Flt-1 14  expressed in endothelial cells is required for normal vascularization.	bind
20808	1	6595	5	NULL	NULL	0	NULL	VEGF-D	NULL		is a ligand for	NULL				VEGFR-2	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_1_11_s_74	9665459	13  VEGF-D is a ligand for both VEGFR-2 and VEGFR-3, but does not bind to the VEGFR-1.	bind
20810	2	6595	5	NULL	NULL	0	NULL	VEGF-D	NULL		is a ligand for	NULL				VEGFR-3	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_1_11_s_74	9665459	13  VEGF-D is a ligand for both VEGFR-2 and VEGFR-3, but does not bind to the VEGFR-1.	bind
20811	3	6595	5	NULL	NULL	0	NULL	VEGF-D	NULL		does not bind	NULL				VEGFR-1	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_1_11_s_74	9665459	13  VEGF-D is a ligand for both VEGFR-2 and VEGFR-3, but does not bind to the VEGFR-1.	bind
25135	1	6595	7	NULL	NULL	NULL	NULL	VEGF-D	GP		is a ligand for					VEGFR-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_1_11_s_74	9665459	13  VEGF-D is a ligand for both VEGFR-2 and VEGFR-3, but does not bind to the VEGFR-1.	bind
25136	2	6595	7	NULL	NULL	NULL	NULL	VEGF-D	GP		is a ligand for					VEGFR-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_1_11_s_74	9665459	13  VEGF-D is a ligand for both VEGFR-2 and VEGFR-3, but does not bind to the VEGFR-1.	bind
25137	3	6595	7	NULL	NULL	NULL	NULL	VEGF-D	GP		does not bind					VEGFR-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_1_11_s_74	9665459	13  VEGF-D is a ligand for both VEGFR-2 and VEGFR-3, but does not bind to the VEGFR-1.	bind
20812	1	6597	5	NULL	NULL	0	NULL	LPS	NULL		bind	NULL				CD14	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_20_2608_s_32	12427659	13 -  15 In vitro studies indicate that the strong proinflammatory response of monocyte/macrophages and neutrophils to LPS requires binding of LPS to CD14 and, at a minimum, TLR4/MD2 for signaling.	bind
20815	2	6597	5	NULL	NULL	0	NULL	LPS	NULL		induces	NULL				proinflammatory response	NULL	strong			NULL	monocyte/macrophages in vitro	NULL	NULL	NULL	NULL	gw60_circulation_106_20_2608_s_32	12427659	13 -  15 In vitro studies indicate that the strong proinflammatory response of monocyte/macrophages and neutrophils to LPS requires binding of LPS to CD14 and, at a minimum, TLR4/MD2 for signaling.	bind
20816	3	6597	5	NULL	NULL	0	NULL	LPS	NULL		induces	NULL				proinflammatory response	NULL	strong			NULL	neutrophils in vitro	NULL	NULL	NULL	NULL	gw60_circulation_106_20_2608_s_32	12427659	13 -  15 In vitro studies indicate that the strong proinflammatory response of monocyte/macrophages and neutrophils to LPS requires binding of LPS to CD14 and, at a minimum, TLR4/MD2 for signaling.	bind
20817	4	6597	5	NULL	NULL	0	NULL	statement 2	NULL		requires	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_20_2608_s_32	12427659	13 -  15 In vitro studies indicate that the strong proinflammatory response of monocyte/macrophages and neutrophils to LPS requires binding of LPS to CD14 and, at a minimum, TLR4/MD2 for signaling.	bind
20818	5	6597	5	NULL	NULL	0	NULL	statement 3	NULL		requires	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_20_2608_s_32	12427659	13 -  15 In vitro studies indicate that the strong proinflammatory response of monocyte/macrophages and neutrophils to LPS requires binding of LPS to CD14 and, at a minimum, TLR4/MD2 for signaling.	bind
20819	6	6597	5	10	NULL	0	NULL	statement 2			requires					TLR4/MD2		signaling of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_20_2608_s_32	12427659	13 -  15 In vitro studies indicate that the strong proinflammatory response of monocyte/macrophages and neutrophils to LPS requires binding of LPS to CD14 and, at a minimum, TLR4/MD2 for signaling.	bind
20820	7	6597	5	10	NULL	0	NULL	statement 3			requires					TLR4/MD2		signaling of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_20_2608_s_32	12427659	13 -  15 In vitro studies indicate that the strong proinflammatory response of monocyte/macrophages and neutrophils to LPS requires binding of LPS to CD14 and, at a minimum, TLR4/MD2 for signaling.	bind
25322	1	6597	7	NULL	NULL	NULL	NULL	LPS	Chemical		bind					CD14	Cell				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulation_106_20_2608_s_32	12427659	13 -  15 In vitro studies indicate that the strong proinflammatory response of monocyte/macrophages and neutrophils to LPS requires binding of LPS to CD14 and, at a minimum, TLR4/MD2 for signaling.	bind
25323	3	6597	7	NULL	NULL	NULL	NULL	statement 2	Process		requires					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_20_2608_s_32	12427659	13 -  15 In vitro studies indicate that the strong proinflammatory response of monocyte/macrophages and neutrophils to LPS requires binding of LPS to CD14 and, at a minimum, TLR4/MD2 for signaling.	bind
25324	5	6597	7	NULL	NULL	NULL	NULL	statement 4	Process		requires					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_20_2608_s_32	12427659	13 -  15 In vitro studies indicate that the strong proinflammatory response of monocyte/macrophages and neutrophils to LPS requires binding of LPS to CD14 and, at a minimum, TLR4/MD2 for signaling.	bind
25325	6	6597	7	NULL	NULL	NULL	NULL	statement 2	Process		requires					TLR4/MD2 	GP	signaling of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulation_106_20_2608_s_32	12427659	13 -  15 In vitro studies indicate that the strong proinflammatory response of monocyte/macrophages and neutrophils to LPS requires binding of LPS to CD14 and, at a minimum, TLR4/MD2 for signaling.	bind
25326	7	6597	7	NULL	NULL	NULL	NULL	statement 4	Process		requires					TLR4/MD2 	GP	signaling of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulation_106_20_2608_s_32	12427659	13 -  15 In vitro studies indicate that the strong proinflammatory response of monocyte/macrophages and neutrophils to LPS requires binding of LPS to CD14 and, at a minimum, TLR4/MD2 for signaling.	bind
25327	2	6597	7	NULL	NULL	NULL	NULL	LPS	Chemical		induces		strong			proinflammatory response	Process				NULL	monocyte/macrophages, in vitro	NULL	NULL	NULL	NULL	gw60_circulation_106_20_2608_s_32	12427659	13 -  15 In vitro studies indicate that the strong proinflammatory response of monocyte/macrophages and neutrophils to LPS requires binding of LPS to CD14 and, at a minimum, TLR4/MD2 for signaling.	bind
25328	4	6597	7	NULL	NULL	NULL	NULL	LPS	Chemical		induces		strong			proinflammatory response	Process				NULL	neutrophils, in vitro	NULL	NULL	NULL	NULL	gw60_circulation_106_20_2608_s_32	12427659	13 -  15 In vitro studies indicate that the strong proinflammatory response of monocyte/macrophages and neutrophils to LPS requires binding of LPS to CD14 and, at a minimum, TLR4/MD2 for signaling.	bind
20821	1	6598	5	10	NULL	0	NULL	GATA-6			bind					SM-MHC		rat;;conserved		GATA-like motif within promoter	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_404_s_23	12615657	13 -  15 We have recently demonstrated that GATA-6 binds a conserved GATA-like motif within the rat SM-MHC promoter and activates this promoter in a sequence-specific manner.	bind
20823	2	6598	5	10	NULL	0	NULL	statement 1			activates		sequence specifically			SM-MHC 		rat		promoter	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_404_s_23	12615657	13 -  15 We have recently demonstrated that GATA-6 binds a conserved GATA-like motif within the rat SM-MHC promoter and activates this promoter in a sequence-specific manner.	bind
25329	1	6598	7	NULL	NULL	NULL	NULL	GATA-6	GP		binds					SM-MHC	GP	rat;;conserved		GATA-like motif within the promoter	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_404_s_23	12615657	13 -  15 We have recently demonstrated that GATA-6 binds a conserved GATA-like motif within the rat SM-MHC promoter and activates this promoter in a sequence-specific manner.	bind
25330	2	6598	7	NULL	NULL	NULL	NULL	statement 1	Process		activates		sequence specifically			SM-MHC	GP	rat		promoter	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_404_s_23	12615657	13 -  15 We have recently demonstrated that GATA-6 binds a conserved GATA-like motif within the rat SM-MHC promoter and activates this promoter in a sequence-specific manner.	bind
20854	1	6599	5	NULL	NULL	0	NULL	platelet subpopulations	NULL		contains	NULL				FV	NULL	distinct levels of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_861_s_28	15653564	13 - 16    Previous studies have shown that the combination of convulxin, a GPVI agonist, and thrombin leads to 2 platelet subpopulations with distinct levels of alpha-granule factor V (FV), and this may be related to serotonin and fibrinogen binding.	bind
20856	2	6599	5	NULL	NULL	0	NULL	FV	NULL		is	NULL				alpha-granule factor V	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_861_s_28	15653564	13 - 16    Previous studies have shown that the combination of convulxin, a GPVI agonist, and thrombin leads to 2 platelet subpopulations with distinct levels of alpha-granule factor V (FV), and this may be related to serotonin and fibrinogen binding.	bind
20857	3	6599	5	NULL	NULL	0	NULL	convulxin	NULL		leads to	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_861_s_28	15653564	13 - 16    Previous studies have shown that the combination of convulxin, a GPVI agonist, and thrombin leads to 2 platelet subpopulations with distinct levels of alpha-granule factor V (FV), and this may be related to serotonin and fibrinogen binding.	bind
20858	4	6599	5	NULL	NULL	0	NULL	convulxin	NULL		is a type of	NULL				GPVI agonist	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_861_s_28	15653564	13 - 16    Previous studies have shown that the combination of convulxin, a GPVI agonist, and thrombin leads to 2 platelet subpopulations with distinct levels of alpha-granule factor V (FV), and this may be related to serotonin and fibrinogen binding.	bind
20859	5	6599	5	NULL	NULL	0	NULL	thrombin	NULL		leads to	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_861_s_28	15653564	13 - 16    Previous studies have shown that the combination of convulxin, a GPVI agonist, and thrombin leads to 2 platelet subpopulations with distinct levels of alpha-granule factor V (FV), and this may be related to serotonin and fibrinogen binding.	bind
20860	6	6599	5	10	NULL	0	NULL	statement 3			occurs in combination with					statement 5					NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_861_s_28	15653564	13 - 16    Previous studies have shown that the combination of convulxin, a GPVI agonist, and thrombin leads to 2 platelet subpopulations with distinct levels of alpha-granule factor V (FV), and this may be related to serotonin and fibrinogen binding.	bind
20861	7	6599	5	10	NULL	0	NULL	statement 6			related to		may be			fibrinogen		binding of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_861_s_28	15653564	13 - 16    Previous studies have shown that the combination of convulxin, a GPVI agonist, and thrombin leads to 2 platelet subpopulations with distinct levels of alpha-granule factor V (FV), and this may be related to serotonin and fibrinogen binding.	bind
20866	8	6599	5	10	NULL	0	NULL	statement 6			related to		may be			serotonin		binding of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_861_s_28	15653564	13 - 16    Previous studies have shown that the combination of convulxin, a GPVI agonist, and thrombin leads to 2 platelet subpopulations with distinct levels of alpha-granule factor V (FV), and this may be related to serotonin and fibrinogen binding.	bind
25331	1	6599	7	NULL	NULL	NULL	NULL	Platelet subpopulations	Cell		contain					FV	GP	distinct levels of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_861_s_28	15653564	13 - 16    Previous studies have shown that the combination of convulxin, a GPVI agonist, and thrombin leads to 2 platelet subpopulations with distinct levels of alpha-granule factor V (FV), and this may be related to serotonin and fibrinogen binding.	bind
25332	4	6599	7	NULL	NULL	NULL	NULL	thrombin	GP		leads to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_861_s_28	15653564	13 - 16    Previous studies have shown that the combination of convulxin, a GPVI agonist, and thrombin leads to 2 platelet subpopulations with distinct levels of alpha-granule factor V (FV), and this may be related to serotonin and fibrinogen binding.	bind
25333	5	6599	7	NULL	NULL	NULL	NULL	statement 2	Process		occurs in combination with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_861_s_28	15653564	13 - 16    Previous studies have shown that the combination of convulxin, a GPVI agonist, and thrombin leads to 2 platelet subpopulations with distinct levels of alpha-granule factor V (FV), and this may be related to serotonin and fibrinogen binding.	bind
25334	6	6599	7	NULL	NULL	NULL	NULL	FV	GP		is					alpha-granule factor V	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_861_s_28	15653564	13 - 16    Previous studies have shown that the combination of convulxin, a GPVI agonist, and thrombin leads to 2 platelet subpopulations with distinct levels of alpha-granule factor V (FV), and this may be related to serotonin and fibrinogen binding.	bind
25336	7	6599	7	NULL	NULL	NULL	NULL	statement 5	Process		be related to		may			serotonin	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_861_s_28	15653564	13 - 16    Previous studies have shown that the combination of convulxin, a GPVI agonist, and thrombin leads to 2 platelet subpopulations with distinct levels of alpha-granule factor V (FV), and this may be related to serotonin and fibrinogen binding.	bind
25859	2	6599	7	NULL	NULL	NULL	NULL	convulxin	GP		leads to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_861_s_28	15653564	13 - 16    Previous studies have shown that the combination of convulxin, a GPVI agonist, and thrombin leads to 2 platelet subpopulations with distinct levels of alpha-granule factor V (FV), and this may be related to serotonin and fibrinogen binding.	bind
25860	3	6599	7	NULL	NULL	NULL	NULL	convulxin	GP		is a type of					GPVI agonist	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_861_s_28	15653564	13 - 16    Previous studies have shown that the combination of convulxin, a GPVI agonist, and thrombin leads to 2 platelet subpopulations with distinct levels of alpha-granule factor V (FV), and this may be related to serotonin and fibrinogen binding.	bind
25861	8	6599	7	NULL	NULL	NULL	NULL	statement 5	Process		be related to		may			fibrinogen	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_861_s_28	15653564	13 - 16    Previous studies have shown that the combination of convulxin, a GPVI agonist, and thrombin leads to 2 platelet subpopulations with distinct levels of alpha-granule factor V (FV), and this may be related to serotonin and fibrinogen binding.	bind
20825	1	6600	5	13	NULL	NULL	NULL	myosin subfragments	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_6_661_s_27	9742062	13 14  In support of this hypothesis was the finding that the binding of myosin subfragments to actin is enhanced in the presence of caldesmon.	bind
20826	2	6600	5	13	NULL	NULL	NULL	caldesmon	GP		enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_6_661_s_27	9742062	13 14  In support of this hypothesis was the finding that the binding of myosin subfragments to actin is enhanced in the presence of caldesmon.	bind
67196	1	6600	5	13	NULL	NULL	NULL	myosin subfragments	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_6_661_s_27	9742062	13 14  In support of this hypothesis was the finding that the binding of myosin subfragments to actin is enhanced in the presence of caldesmon.	bind
25337	1	6600	7	NULL	NULL	NULL	NULL	myosin subfragments	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_6_661_s_27	9742062	13 14  In support of this hypothesis was the finding that the binding of myosin subfragments to actin is enhanced in the presence of caldesmon.	bind
25338	2	6600	7	13	NULL	NULL	NULL	caldesmon	GP		enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_6_661_s_27	9742062	13 14  In support of this hypothesis was the finding that the binding of myosin subfragments to actin is enhanced in the presence of caldesmon.	bind
20869	1	6601	5	13	NULL	NULL	NULL	OPN	GP		bind		directly			collagen I	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_10_1080_s_229	11375279	13 14  In the models of skin incision/wound healing and in obstructive uropathy, disorganization of collagen and decreases in collagen I content were observed in mice lacking OPN. 13 14  OPN can bind directly to collagen I and interacts with collagen II, III, IV, V, and fibronectin.	bind
20870	2	6601	5	13	NULL	NULL	NULL	OPN	GP		interacts with					collagen II	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_10_1080_s_229	11375279	13 14  In the models of skin incision/wound healing and in obstructive uropathy, disorganization of collagen and decreases in collagen I content were observed in mice lacking OPN. 13 14  OPN can bind directly to collagen I and interacts with collagen II, III, IV, V, and fibronectin.	bind
20871	3	6601	5	13	NULL	NULL	NULL	OPN	GP		interacts with					collagen III	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_10_1080_s_229	11375279	13 14  In the models of skin incision/wound healing and in obstructive uropathy, disorganization of collagen and decreases in collagen I content were observed in mice lacking OPN. 13 14  OPN can bind directly to collagen I and interacts with collagen II, III, IV, V, and fibronectin.	bind
20872	4	6601	5	13	NULL	NULL	NULL	OPN	GP		interacts with					collagen IV	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_10_1080_s_229	11375279	13 14  In the models of skin incision/wound healing and in obstructive uropathy, disorganization of collagen and decreases in collagen I content were observed in mice lacking OPN. 13 14  OPN can bind directly to collagen I and interacts with collagen II, III, IV, V, and fibronectin.	bind
20873	5	6601	5	13	NULL	NULL	NULL	OPN	GP		interacts with					collagen V	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_10_1080_s_229	11375279	13 14  In the models of skin incision/wound healing and in obstructive uropathy, disorganization of collagen and decreases in collagen I content were observed in mice lacking OPN. 13 14  OPN can bind directly to collagen I and interacts with collagen II, III, IV, V, and fibronectin.	bind
20874	6	6601	5	13	NULL	NULL	NULL	OPN	GP		interacts with					fibronectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_10_1080_s_229	11375279	13 14  In the models of skin incision/wound healing and in obstructive uropathy, disorganization of collagen and decreases in collagen I content were observed in mice lacking OPN. 13 14  OPN can bind directly to collagen I and interacts with collagen II, III, IV, V, and fibronectin.	bind
56119	7	6601	5	13	NULL	NULL	NULL	collagen	GP		is disorganized in					OPN	GP	mice lacking			NULL	models of skin incision/wound healing	NULL	NULL	NULL	NULL	gw60_circulationres_88_10_1080_s_229	11375279	13 14  In the models of skin incision/wound healing and in obstructive uropathy, disorganization of collagen and decreases in collagen I content were observed in mice lacking OPN. 13 14  OPN can bind directly to collagen I and interacts with collagen II, III, IV, V, and fibronectin.	bind
56120	8	6601	5	13	NULL	NULL	NULL	collagen	GP		is disorganized in					OPN	GP	mice lacking			NULL	obstructive uropathy	NULL	NULL	NULL	NULL	gw60_circulationres_88_10_1080_s_229	11375279	13 14  In the models of skin incision/wound healing and in obstructive uropathy, disorganization of collagen and decreases in collagen I content were observed in mice lacking OPN. 13 14  OPN can bind directly to collagen I and interacts with collagen II, III, IV, V, and fibronectin.	bind
56121	9	6601	5	13	NULL	NULL	NULL	collagen I	GP		decrease in					OPN	GP	mice lacking			NULL	models of skin incision/wound healing	NULL	NULL	NULL	NULL	gw60_circulationres_88_10_1080_s_229	11375279	13 14  In the models of skin incision/wound healing and in obstructive uropathy, disorganization of collagen and decreases in collagen I content were observed in mice lacking OPN. 13 14  OPN can bind directly to collagen I and interacts with collagen II, III, IV, V, and fibronectin.	bind
56122	10	6601	5	13	NULL	NULL	NULL	collagen	GP		decrease in					OPN	GP	mice lacking			NULL	obstructive uropathy	NULL	NULL	NULL	NULL	gw60_circulationres_88_10_1080_s_229	11375279	13 14  In the models of skin incision/wound healing and in obstructive uropathy, disorganization of collagen and decreases in collagen I content were observed in mice lacking OPN. 13 14  OPN can bind directly to collagen I and interacts with collagen II, III, IV, V, and fibronectin.	bind
18532	1	6601	6	13	NULL	NULL	NULL	OPN	GP		bind		directly			collagen I	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_10_1080_s_229	11375279	13 14  In the models of skin incision/wound healing and in obstructive uropathy, disorganization of collagen and decreases in collagen I content were observed in mice lacking OPN. 13 14  OPN can bind directly to collagen I and interacts with collagen II, III, IV, V, and fibronectin.	bind
18533	2	6601	6	13	NULL	NULL	NULL	OPN	GP		interacts with					collagen II	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_10_1080_s_229	11375279	13 14  In the models of skin incision/wound healing and in obstructive uropathy, disorganization of collagen and decreases in collagen I content were observed in mice lacking OPN. 13 14  OPN can bind directly to collagen I and interacts with collagen II, III, IV, V, and fibronectin.	bind
18534	3	6601	6	13	NULL	NULL	NULL	OPN	GP		interacts with					collagen III	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_10_1080_s_229	11375279	13 14  In the models of skin incision/wound healing and in obstructive uropathy, disorganization of collagen and decreases in collagen I content were observed in mice lacking OPN. 13 14  OPN can bind directly to collagen I and interacts with collagen II, III, IV, V, and fibronectin.	bind
18535	4	6601	6	13	NULL	NULL	NULL	OPN	GP		interacts with					collagen IV	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_10_1080_s_229	11375279	13 14  In the models of skin incision/wound healing and in obstructive uropathy, disorganization of collagen and decreases in collagen I content were observed in mice lacking OPN. 13 14  OPN can bind directly to collagen I and interacts with collagen II, III, IV, V, and fibronectin.	bind
18536	5	6601	6	13	NULL	NULL	NULL	OPN	GP		interacts with					collagen V	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_10_1080_s_229	11375279	13 14  In the models of skin incision/wound healing and in obstructive uropathy, disorganization of collagen and decreases in collagen I content were observed in mice lacking OPN. 13 14  OPN can bind directly to collagen I and interacts with collagen II, III, IV, V, and fibronectin.	bind
18537	6	6601	6	13	NULL	NULL	NULL	OPN	GP		interacts with					fibronectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_10_1080_s_229	11375279	13 14  In the models of skin incision/wound healing and in obstructive uropathy, disorganization of collagen and decreases in collagen I content were observed in mice lacking OPN. 13 14  OPN can bind directly to collagen I and interacts with collagen II, III, IV, V, and fibronectin.	bind
56123	7	6601	6	13	NULL	NULL	NULL	collagen	GP		is disorganized in					OPN	GP	mice lacking			NULL	models of skin incision/wound healing	NULL	NULL	NULL	NULL	gw60_circulationres_88_10_1080_s_229	11375279	13 14  In the models of skin incision/wound healing and in obstructive uropathy, disorganization of collagen and decreases in collagen I content were observed in mice lacking OPN. 13 14  OPN can bind directly to collagen I and interacts with collagen II, III, IV, V, and fibronectin.	bind
56124	8	6601	6	13	NULL	NULL	NULL	collagen	GP		is disorganized in					OPN	GP	mice lacking			NULL	obstructive uropathy	NULL	NULL	NULL	NULL	gw60_circulationres_88_10_1080_s_229	11375279	13 14  In the models of skin incision/wound healing and in obstructive uropathy, disorganization of collagen and decreases in collagen I content were observed in mice lacking OPN. 13 14  OPN can bind directly to collagen I and interacts with collagen II, III, IV, V, and fibronectin.	bind
56125	9	6601	6	13	NULL	NULL	NULL	collagen I	GP		decrease in					OPN	GP	mice lacking			NULL	models of skin incision/wound healing	NULL	NULL	NULL	NULL	gw60_circulationres_88_10_1080_s_229	11375279	13 14  In the models of skin incision/wound healing and in obstructive uropathy, disorganization of collagen and decreases in collagen I content were observed in mice lacking OPN. 13 14  OPN can bind directly to collagen I and interacts with collagen II, III, IV, V, and fibronectin.	bind
56126	10	6601	6	13	NULL	NULL	NULL	collagen I	GP		decrease in					OPN	GP	mice lacking			NULL	obstructive uropathy	NULL	NULL	NULL	NULL	gw60_circulationres_88_10_1080_s_229	11375279	13 14  In the models of skin incision/wound healing and in obstructive uropathy, disorganization of collagen and decreases in collagen I content were observed in mice lacking OPN. 13 14  OPN can bind directly to collagen I and interacts with collagen II, III, IV, V, and fibronectin.	bind
18663	1	6602	6	13	NULL	NULL	NULL	NAD(H)	Chemical		bind					IDH2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_2_1204_s_215	11042198	13 and  14; summarized in Table  III) consistent with these designations of catalytic  versus regulatory function include ( a) substitutions for active site serine residues corresponding to bacterial Ser-113 that reduce catalytic activity (IDH2 S98A)  versus cooperativity and AMP activation (IDH1 S92A) and ( b) substitutions for adjacent residues corresponding to bacterial residues known to be important for cofactor specificity ( 25) that eliminate apparent binding of NAD(H) by IDH2 (D286A/I287A)  versus of AMP by IDH1 (D279A/I280A).	bind
18664	2	6602	6	13	NULL	NULL	NULL			substitution of	eliminates			D286A/I287A		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_2_1204_s_215	11042198	13 and  14; summarized in Table  III) consistent with these designations of catalytic  versus regulatory function include ( a) substitutions for active site serine residues corresponding to bacterial Ser-113 that reduce catalytic activity (IDH2 S98A)  versus cooperativity and AMP activation (IDH1 S92A) and ( b) substitutions for adjacent residues corresponding to bacterial residues known to be important for cofactor specificity ( 25) that eliminate apparent binding of NAD(H) by IDH2 (D286A/I287A)  versus of AMP by IDH1 (D279A/I280A).	bind
18740	3	6602	6	13	NULL	NULL	NULL	AMP	Chemical		bind					IDH1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_2_1204_s_215	11042198	13 and  14; summarized in Table  III) consistent with these designations of catalytic  versus regulatory function include ( a) substitutions for active site serine residues corresponding to bacterial Ser-113 that reduce catalytic activity (IDH2 S98A)  versus cooperativity and AMP activation (IDH1 S92A) and ( b) substitutions for adjacent residues corresponding to bacterial residues known to be important for cofactor specificity ( 25) that eliminate apparent binding of NAD(H) by IDH2 (D286A/I287A)  versus of AMP by IDH1 (D279A/I280A).	bind
18741	4	6602	6	13	NULL	NULL	NULL			substitution of	eliminates			D279A/I280A		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_2_1204_s_215	11042198	13 and  14; summarized in Table  III) consistent with these designations of catalytic  versus regulatory function include ( a) substitutions for active site serine residues corresponding to bacterial Ser-113 that reduce catalytic activity (IDH2 S98A)  versus cooperativity and AMP activation (IDH1 S92A) and ( b) substitutions for adjacent residues corresponding to bacterial residues known to be important for cofactor specificity ( 25) that eliminate apparent binding of NAD(H) by IDH2 (D286A/I287A)  versus of AMP by IDH1 (D279A/I280A).	bind
24750	1	6603	5	13	NULL	NULL	NULL	MyBP-C	GP		modulates					myosin crossbridges	CellComponent	range of movement of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_8_752_s_140	14500336	13 Based on these results, a model was proposed in which MyBP-C modulates the range of movement of myosin crossbridges, perhaps by tethering the crossbridges to the thick filament backbone, so that following MyBP-C extraction crossbridges are less constrained and the probability of myosin binding to actin is increased.	bind
24752	2	6603	5	13	NULL	NULL	NULL	myosin crossbridges	CellComponent		is tethered to					filament backbone	CellComponent	thick			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_8_752_s_140	14500336	13 Based on these results, a model was proposed in which MyBP-C modulates the range of movement of myosin crossbridges, perhaps by tethering the crossbridges to the thick filament backbone, so that following MyBP-C extraction crossbridges are less constrained and the probability of myosin binding to actin is increased.	bind
24753	3	6603	5	13	NULL	NULL	NULL	statement 1	Process		occurs by		perhaps			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_8_752_s_140	14500336	13 Based on these results, a model was proposed in which MyBP-C modulates the range of movement of myosin crossbridges, perhaps by tethering the crossbridges to the thick filament backbone, so that following MyBP-C extraction crossbridges are less constrained and the probability of myosin binding to actin is increased.	bind
24754	4	6603	5	13	NULL	NULL	NULL	MyBP-C	GP	extraction of	leads to					crossbridges	CellComponent	less constrained			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_8_752_s_140	14500336	13 Based on these results, a model was proposed in which MyBP-C modulates the range of movement of myosin crossbridges, perhaps by tethering the crossbridges to the thick filament backbone, so that following MyBP-C extraction crossbridges are less constrained and the probability of myosin binding to actin is increased.	bind
24755	5	6603	5	13	NULL	NULL	NULL	myosin	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_8_752_s_140	14500336	13 Based on these results, a model was proposed in which MyBP-C modulates the range of movement of myosin crossbridges, perhaps by tethering the crossbridges to the thick filament backbone, so that following MyBP-C extraction crossbridges are less constrained and the probability of myosin binding to actin is increased.	bind
24756	6	6603	5	13	NULL	NULL	NULL	MyBP-C	GP	extraction of	leads to					statement 5	Process	increased probability of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_8_752_s_140	14500336	13 Based on these results, a model was proposed in which MyBP-C modulates the range of movement of myosin crossbridges, perhaps by tethering the crossbridges to the thick filament backbone, so that following MyBP-C extraction crossbridges are less constrained and the probability of myosin binding to actin is increased.	bind
18541	1	6603	6	13	NULL	NULL	NULL	myosin	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_8_752_s_140	14500336	13 Based on these results, a model was proposed in which MyBP-C modulates the range of movement of myosin crossbridges, perhaps by tethering the crossbridges to the thick filament backbone, so that following MyBP-C extraction crossbridges are less constrained and the probability of myosin binding to actin is increased.	bind
30284	2	6603	6	13	NULL	NULL	NULL	MyBP-C	GP		modulates		may			myosin crossbridges	CellComponent	range of movement of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_8_752_s_140	14500336	13 Based on these results, a model was proposed in which MyBP-C modulates the range of movement of myosin crossbridges, perhaps by tethering the crossbridges to the thick filament backbone, so that following MyBP-C extraction crossbridges are less constrained and the probability of myosin binding to actin is increased.	bind
30285	3	6603	6	13	NULL	NULL	NULL	myosin crossbridges	CellComponent		are tethered to		perhaps			filament backbone	CellComponent	thick			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_8_752_s_140	14500336	13 Based on these results, a model was proposed in which MyBP-C modulates the range of movement of myosin crossbridges, perhaps by tethering the crossbridges to the thick filament backbone, so that following MyBP-C extraction crossbridges are less constrained and the probability of myosin binding to actin is increased.	bind
30286	4	6603	6	13	NULL	NULL	NULL	MyBP-C	GP		modulates					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_8_752_s_140	14500336	13 Based on these results, a model was proposed in which MyBP-C modulates the range of movement of myosin crossbridges, perhaps by tethering the crossbridges to the thick filament backbone, so that following MyBP-C extraction crossbridges are less constrained and the probability of myosin binding to actin is increased.	bind
30311	5	6603	6	13	NULL	NULL	NULL	MyBP-C	GP	extraction of	leads to					crossbridges	CellComponent	less constrained			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_8_752_s_140	14500336	13 Based on these results, a model was proposed in which MyBP-C modulates the range of movement of myosin crossbridges, perhaps by tethering the crossbridges to the thick filament backbone, so that following MyBP-C extraction crossbridges are less constrained and the probability of myosin binding to actin is increased.	bind
56131	6	6603	6	13	NULL	NULL	NULL	MyBP-C	GP	extraction of	increase					statement 1	Process	probability of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_8_752_s_140	14500336	13 Based on these results, a model was proposed in which MyBP-C modulates the range of movement of myosin crossbridges, perhaps by tethering the crossbridges to the thick filament backbone, so that following MyBP-C extraction crossbridges are less constrained and the probability of myosin binding to actin is increased.	bind
24757	1	6604	5	13	NULL	NULL	NULL	PAI-1	GP	mutant	bind		normally			vitronectin	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_365_s_157	15576638	13 In an experimental model of glomerulonephritis, intravenous administration of a mutant PAI-1 that binds vitronectin normally but lacks protease inhibitory activity, restored plasmin generation, and reduced matrix accumulation of collagen I, collagen III, fibronectin, and laminin.	bind
24758	2	6604	5	13	NULL	NULL	NULL	PAI-1	GP	mutant	lacks					protease inhibitory activity					NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_365_s_157	15576638	13 In an experimental model of glomerulonephritis, intravenous administration of a mutant PAI-1 that binds vitronectin normally but lacks protease inhibitory activity, restored plasmin generation, and reduced matrix accumulation of collagen I, collagen III, fibronectin, and laminin.	bind
24759	3	6604	5	13	NULL	NULL	NULL	PAI-1	GP	mutant	restored					plasmin	GP	generation of			NULL	in an experimental model of glomerulonephritis	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_365_s_157	15576638	13 In an experimental model of glomerulonephritis, intravenous administration of a mutant PAI-1 that binds vitronectin normally but lacks protease inhibitory activity, restored plasmin generation, and reduced matrix accumulation of collagen I, collagen III, fibronectin, and laminin.	bind
24760	4	6604	5	13	NULL	NULL	NULL	PAI-1	GP	mutant	reduces					collagen I	GP	matrix accumulation of			NULL	in an experimental model of glomerulonephritis	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_365_s_157	15576638	13 In an experimental model of glomerulonephritis, intravenous administration of a mutant PAI-1 that binds vitronectin normally but lacks protease inhibitory activity, restored plasmin generation, and reduced matrix accumulation of collagen I, collagen III, fibronectin, and laminin.	bind
24761	5	6604	5	13	NULL	NULL	NULL	PAI-1	GP	mutant	reduces					collagen III	GP	matrix accumulation of			NULL	in an experimental model of glomerulonephritis	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_365_s_157	15576638	13 In an experimental model of glomerulonephritis, intravenous administration of a mutant PAI-1 that binds vitronectin normally but lacks protease inhibitory activity, restored plasmin generation, and reduced matrix accumulation of collagen I, collagen III, fibronectin, and laminin.	bind
24762	6	6604	5	13	NULL	NULL	NULL	PAI-1	GP	mutant	reduces					fibronectin	GP	matrix accumulation of			NULL	in an experimental model of glomerulonephritis	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_365_s_157	15576638	13 In an experimental model of glomerulonephritis, intravenous administration of a mutant PAI-1 that binds vitronectin normally but lacks protease inhibitory activity, restored plasmin generation, and reduced matrix accumulation of collagen I, collagen III, fibronectin, and laminin.	bind
24763	7	6604	5	13	NULL	NULL	NULL	PAI-1	GP	mutant	reduces					laminin	GP	matrix accumulation of			NULL	in an experimental model of glomerulonephritis	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_365_s_157	15576638	13 In an experimental model of glomerulonephritis, intravenous administration of a mutant PAI-1 that binds vitronectin normally but lacks protease inhibitory activity, restored plasmin generation, and reduced matrix accumulation of collagen I, collagen III, fibronectin, and laminin.	bind
18543	1	6604	6	13	NULL	NULL	NULL	PAI-1	GP	mutant	bind					vitronectin	GP				NULL	experimental model of glomerulonephritis	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_365_s_157	15576638	13 In an experimental model of glomerulonephritis, intravenous administration of a mutant PAI-1 that binds vitronectin normally but lacks protease inhibitory activity, restored plasmin generation, and reduced matrix accumulation of collagen I, collagen III, fibronectin, and laminin.	bind
18598	2	6604	6	13	NULL	NULL	NULL	PAI-1	GP	mutant	lacks					protease inhibitory activity					NULL	experimental model of glomerulonephritis	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_365_s_157	15576638	13 In an experimental model of glomerulonephritis, intravenous administration of a mutant PAI-1 that binds vitronectin normally but lacks protease inhibitory activity, restored plasmin generation, and reduced matrix accumulation of collagen I, collagen III, fibronectin, and laminin.	bind
18599	3	6604	6	13	NULL	NULL	NULL	PAI-1	GP	mutant	restored					plasmin	GP	generation of			NULL	experimental model of glomerulonephritis	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_365_s_157	15576638	13 In an experimental model of glomerulonephritis, intravenous administration of a mutant PAI-1 that binds vitronectin normally but lacks protease inhibitory activity, restored plasmin generation, and reduced matrix accumulation of collagen I, collagen III, fibronectin, and laminin.	bind
18600	4	6604	6	13	NULL	NULL	NULL	PAI-1	GP	mutant	reduced					collagen I	GP	matrix accumulation of 			NULL	experimental model of glomerulonephritis	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_365_s_157	15576638	13 In an experimental model of glomerulonephritis, intravenous administration of a mutant PAI-1 that binds vitronectin normally but lacks protease inhibitory activity, restored plasmin generation, and reduced matrix accumulation of collagen I, collagen III, fibronectin, and laminin.	bind
18601	5	6604	6	13	NULL	NULL	NULL	PAI-1	GP	mutant	reduced					collagen III	GP	matrix accumulation of			NULL	experimental model of glomerulonephritis	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_365_s_157	15576638	13 In an experimental model of glomerulonephritis, intravenous administration of a mutant PAI-1 that binds vitronectin normally but lacks protease inhibitory activity, restored plasmin generation, and reduced matrix accumulation of collagen I, collagen III, fibronectin, and laminin.	bind
18602	6	6604	6	13	NULL	NULL	NULL	PAI-1	GP	mutant	reduced					fibronectin	GP	matrix accumulation of			NULL	experimental model of glomerulonephritis	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_365_s_157	15576638	13 In an experimental model of glomerulonephritis, intravenous administration of a mutant PAI-1 that binds vitronectin normally but lacks protease inhibitory activity, restored plasmin generation, and reduced matrix accumulation of collagen I, collagen III, fibronectin, and laminin.	bind
18603	7	6604	6	13	NULL	NULL	NULL	PAI-1	GP	mutant	reduced					laminin	GP	matrix accumulation of			NULL	experimental model of glomerulonephritis	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_365_s_157	15576638	13 In an experimental model of glomerulonephritis, intravenous administration of a mutant PAI-1 that binds vitronectin normally but lacks protease inhibitory activity, restored plasmin generation, and reduced matrix accumulation of collagen I, collagen III, fibronectin, and laminin.	bind
20879	1	6605	5	13	NULL	NULL	NULL	apoA-I	GP	human	bind					lipid hydroperoxides	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1325_s_57	15831812	13 It was concluded that human apoA-I binds lipid hydroperoxides in such a manner that the lipid hydroperoxides can still participate in the formation of oxidized phospholipids if the apoA-I-lipid hydroperoxide complexes are not removed.	bind
20881	2	6605	5	13	NULL	NULL	NULL	lipid hydroperoxides	Chemical		participate in					oxidized phospholipids	Chemical	formation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1325_s_57	15831812	13 It was concluded that human apoA-I binds lipid hydroperoxides in such a manner that the lipid hydroperoxides can still participate in the formation of oxidized phospholipids if the apoA-I-lipid hydroperoxide complexes are not removed.	bind
20884	3	6605	5	13	NULL	NULL	NULL	statement 2	Process		on non removal of					apoA-I-lipid hydroperoxide complexes	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1325_s_57	15831812	13 It was concluded that human apoA-I binds lipid hydroperoxides in such a manner that the lipid hydroperoxides can still participate in the formation of oxidized phospholipids if the apoA-I-lipid hydroperoxide complexes are not removed.	bind
18604	1	6605	6	13	NULL	NULL	NULL	apoA-I	GP	human	bind					lipid hydroperoxides	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1325_s_57	15831812	13 It was concluded that human apoA-I binds lipid hydroperoxides in such a manner that the lipid hydroperoxides can still participate in the formation of oxidized phospholipids if the apoA-I-lipid hydroperoxide complexes are not removed.	bind
18605	2	6605	6	13	NULL	NULL	NULL	lipid hydroperoxides	Chemical		participate					oxidized phospholipids	Chemical	formation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1325_s_57	15831812	13 It was concluded that human apoA-I binds lipid hydroperoxides in such a manner that the lipid hydroperoxides can still participate in the formation of oxidized phospholipids if the apoA-I-lipid hydroperoxide complexes are not removed.	bind
18606	3	6605	6	13	NULL	NULL	NULL	statement 2	Process		occurs on nonremoval of					apoA-I-lipid hydroperoxide complexes	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1325_s_57	15831812	13 It was concluded that human apoA-I binds lipid hydroperoxides in such a manner that the lipid hydroperoxides can still participate in the formation of oxidized phospholipids if the apoA-I-lipid hydroperoxide complexes are not removed.	bind
20885	1	6606	5	13	NULL	NULL	NULL	plasma constituents	CellComponent		bind					PDGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_24_2893_s_161	12070119	13 Raines et al 29 reported the presence of plasma constituents, which have the capacity to bind to PDGF and inhibit the binding of PDGF to its cell-surface receptor.	bind
20886	2	6606	5	13	NULL	NULL	NULL	PDGF	GP		bind					cell-surface receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_24_2893_s_161	12070119	13 Raines et al 29 reported the presence of plasma constituents, which have the capacity to bind to PDGF and inhibit the binding of PDGF to its cell-surface receptor.	bind
20887	3	6606	5	13	NULL	NULL	NULL	plasma constituents	CellComponent		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_24_2893_s_161	12070119	13 Raines et al 29 reported the presence of plasma constituents, which have the capacity to bind to PDGF and inhibit the binding of PDGF to its cell-surface receptor.	bind
18607	1	6606	6	13	NULL	NULL	NULL	plasma constituents	CellComponent		bind					PDGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_24_2893_s_161	12070119	13 Raines et al 29 reported the presence of plasma constituents, which have the capacity to bind to PDGF and inhibit the binding of PDGF to its cell-surface receptor.	bind
18608	2	6606	6	13	NULL	NULL	NULL	PDGF	GP		bind					cell-surface receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_24_2893_s_161	12070119	13 Raines et al 29 reported the presence of plasma constituents, which have the capacity to bind to PDGF and inhibit the binding of PDGF to its cell-surface receptor.	bind
18609	3	6606	6	13	NULL	NULL	NULL	plasma constituents	CellComponent		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_24_2893_s_161	12070119	13 Raines et al 29 reported the presence of plasma constituents, which have the capacity to bind to PDGF and inhibit the binding of PDGF to its cell-surface receptor.	bind
20888	1	6607	5	13	NULL	NULL	NULL	vitronectin	GP	radiolabeled	bind					fibrin matrices	CellComponent	pre-formed			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_12_2679_s_164	16210568	13 The apparent binding affinity estimated by SPR ( KD of 0.26 mumol/L) is higher but consistent with that previously determined by solid-phase binding assay ( KD of  0.60 mumol/L) in which radiolabeled vitronectin was bound to pre-formed fibrin matrices.	bind
18610	1	6607	6	13	NULL	NULL	NULL	vitronectin	GP	radiolabeled	bind					fibrin matrices	CellComponent	pre-formed 			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_12_2679_s_164	16210568	13 The apparent binding affinity estimated by SPR ( KD of 0.26 mumol/L) is higher but consistent with that previously determined by solid-phase binding assay ( KD of  0.60 mumol/L) in which radiolabeled vitronectin was bound to pre-formed fibrin matrices.	bind
20889	1	6608	5	13	NULL	NULL	NULL	NFAT	GP		bind					calcineurin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_7_725_s_81	12663489	13 The VIVIT peptide was found to be 25 times more effective at inhibiting NFAT binding to calcineurin than a peptide spanning the naturally occurring calcineurin binding site of NFATc2.	bind
20890	2	6608	5	13	NULL	NULL	NULL	VIVIT peptide	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_7_725_s_81	12663489	13 The VIVIT peptide was found to be 25 times more effective at inhibiting NFAT binding to calcineurin than a peptide spanning the naturally occurring calcineurin binding site of NFATc2.	bind
20891	3	6608	5	13	NULL	NULL	NULL	peptide	GP	 naturally occurring 	inhibit			calcineurin binding site of NFATc2		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_7_725_s_81	12663489	13 The VIVIT peptide was found to be 25 times more effective at inhibiting NFAT binding to calcineurin than a peptide spanning the naturally occurring calcineurin binding site of NFATc2.	bind
20892	4	6608	5	13	NULL	NULL	NULL	statement 2	Process		more effective than					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_7_725_s_81	12663489	13 The VIVIT peptide was found to be 25 times more effective at inhibiting NFAT binding to calcineurin than a peptide spanning the naturally occurring calcineurin binding site of NFATc2.	bind
18611	1	6608	6	13	NULL	NULL	NULL	NFAT	GP		bind					calcineurin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_7_725_s_81	12663489	13 The VIVIT peptide was found to be 25 times more effective at inhibiting NFAT binding to calcineurin than a peptide spanning the naturally occurring calcineurin binding site of NFATc2.	bind
18612	2	6608	6	13	NULL	NULL	NULL	VIVIT peptide	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_7_725_s_81	12663489	13 The VIVIT peptide was found to be 25 times more effective at inhibiting NFAT binding to calcineurin than a peptide spanning the naturally occurring calcineurin binding site of NFATc2.	bind
18613	3	6608	6	13	NULL	NULL	NULL	peptide	GP	naturally occuring	inhibits			calcineurin binding site of NFATc2		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_7_725_s_81	12663489	13 The VIVIT peptide was found to be 25 times more effective at inhibiting NFAT binding to calcineurin than a peptide spanning the naturally occurring calcineurin binding site of NFATc2.	bind
30283	4	6608	6	13	NULL	NULL	NULL	statement 2	Process		is more effective than					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_7_725_s_81	12663489	13 The VIVIT peptide was found to be 25 times more effective at inhibiting NFAT binding to calcineurin than a peptide spanning the naturally occurring calcineurin binding site of NFATc2.	bind
20893	1	6609	5	13	NULL	NULL	NULL	Rad	GP		bind					GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_8_1071_s_25	15710763	13 These interactions are enhanced by an increase in calcium influx and favor the inactive GDP-bound form of Rad.	bind
18614	1	6609	6	13	NULL	NULL	NULL	GDP	Chemical		bind					Rad	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_8_1071_s_25	15710763	13 These interactions are enhanced by an increase in calcium influx and favor the inactive GDP-bound form of Rad.	bind
20894	1	6610	5	13	NULL	NULL	NULL	monocytes	Cell	attached	is capable of					LDL	GP	uptake of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_684_s_135	14988094	13 To exclude that these cells are attached monocytes or macrophages, which are also capable for LDL uptake and lectin binding, 17,18  additional characterization is necessary.	bind
20899	2	6610	5	13	NULL	NULL	NULL	macrophages	Cell	attached	is capable of					LDL	GP	uptake of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_684_s_135	14988094	13 To exclude that these cells are attached monocytes or macrophages, which are also capable for LDL uptake and lectin binding, 17,18  additional characterization is necessary.	bind
20900	3	6610	5	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_684_s_135	14988094	13 To exclude that these cells are attached monocytes or macrophages, which are also capable for LDL uptake and lectin binding, 17,18  additional characterization is necessary.	bind
20901	4	6610	5	13	NULL	NULL	NULL	monocytes	Cell	attached	bind					lectin	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_684_s_135	14988094	13 To exclude that these cells are attached monocytes or macrophages, which are also capable for LDL uptake and lectin binding, 17,18  additional characterization is necessary.	bind
20902	5	6610	5	13	NULL	NULL	NULL	macrophages	Cell	attached	bind					lectin	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_684_s_135	14988094	13 To exclude that these cells are attached monocytes or macrophages, which are also capable for LDL uptake and lectin binding, 17,18  additional characterization is necessary.	bind
20903	6	6610	5	13	NULL	NULL	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_684_s_135	14988094	13 To exclude that these cells are attached monocytes or macrophages, which are also capable for LDL uptake and lectin binding, 17,18  additional characterization is necessary.	bind
18615	1	6610	6	13	NULL	NULL	NULL	monocytes	Cell	attached	are capable of					LDL	GP	uptake of 			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_684_s_135	14988094	13 To exclude that these cells are attached monocytes or macrophages, which are also capable for LDL uptake and lectin binding, 17,18  additional characterization is necessary.	bind
18616	2	6610	6	13	NULL	NULL	NULL	monocytes	Cell	attached	bind					lectin	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_684_s_135	14988094	13 To exclude that these cells are attached monocytes or macrophages, which are also capable for LDL uptake and lectin binding, 17,18  additional characterization is necessary.	bind
18617	3	6610	6	13	NULL	NULL	NULL	macrophages	Cell	attached 	bind					lectin	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_684_s_135	14988094	13 To exclude that these cells are attached monocytes or macrophages, which are also capable for LDL uptake and lectin binding, 17,18  additional characterization is necessary.	bind
18618	4	6610	6	13	NULL	NULL	NULL	macrophages	Cell	attached	are capable of					LDL 	GP	uptake of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_684_s_135	14988094	13 To exclude that these cells are attached monocytes or macrophages, which are also capable for LDL uptake and lectin binding, 17,18  additional characterization is necessary.	bind
30281	5	6610	6	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_684_s_135	14988094	13 To exclude that these cells are attached monocytes or macrophages, which are also capable for LDL uptake and lectin binding, 17,18  additional characterization is necessary.	bind
30282	6	6610	6	13	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_684_s_135	14988094	13 To exclude that these cells are attached monocytes or macrophages, which are also capable for LDL uptake and lectin binding, 17,18  additional characterization is necessary.	bind
20904	1	6611	5	13	NULL	NULL	NULL	TTP	GP		bind					TNF-alpha mRNA	NucleicAcid			AU-rich element in 3' untranslated region	NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_17_2631_s_32	15492321	13 TTP binds to the AU-rich element in the 3' untranslated region of TNF-alpha mRNA to destabilize the mRNA. STAT6 signaling has been reported to induce TTP in mast cells, which then reduces the expression of TNF-alpha.	bind
20905	2	6611	5	13	NULL	NULL	NULL	statement 1	Process		destabilize					TNF-alpha mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_17_2631_s_32	15492321	13 TTP binds to the AU-rich element in the 3' untranslated region of TNF-alpha mRNA to destabilize the mRNA. STAT6 signaling has been reported to induce TTP in mast cells, which then reduces the expression of TNF-alpha.	bind
20906	3	6611	5	13	NULL	NULL	NULL	STAT6 signaling	Process		induces					TTP	GP				NULL	in mast cells	NULL	NULL	NULL	NULL	gw70_circulation_110_17_2631_s_32	15492321	13 TTP binds to the AU-rich element in the 3' untranslated region of TNF-alpha mRNA to destabilize the mRNA. STAT6 signaling has been reported to induce TTP in mast cells, which then reduces the expression of TNF-alpha.	bind
20908	4	6611	5	13	NULL	NULL	NULL	statement 3	Process		reduces					TNF-alpha	GP	expression of 			NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_17_2631_s_32	15492321	13 TTP binds to the AU-rich element in the 3' untranslated region of TNF-alpha mRNA to destabilize the mRNA. STAT6 signaling has been reported to induce TTP in mast cells, which then reduces the expression of TNF-alpha.	bind
18619	1	6611	6	13	NULL	NULL	NULL	TTP	GP		bind					TNF-alpha mRNA	NucleicAcid			AU-rich element in 3' untranslated region	NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_17_2631_s_32	15492321	13 TTP binds to the AU-rich element in the 3' untranslated region of TNF-alpha mRNA to destabilize the mRNA. STAT6 signaling has been reported to induce TTP in mast cells, which then reduces the expression of TNF-alpha.	bind
18620	2	6611	6	13	NULL	NULL	NULL	STAT6 signaling	Process		induce					TTP	GP				NULL	mast cells	NULL	NULL	NULL	NULL	gw70_circulation_110_17_2631_s_32	15492321	13 TTP binds to the AU-rich element in the 3' untranslated region of TNF-alpha mRNA to destabilize the mRNA. STAT6 signaling has been reported to induce TTP in mast cells, which then reduces the expression of TNF-alpha.	bind
18621	3	6611	6	13	NULL	NULL	NULL	STAT6 signaling	Process		reduces					TNF-alpha	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_17_2631_s_32	15492321	13 TTP binds to the AU-rich element in the 3' untranslated region of TNF-alpha mRNA to destabilize the mRNA. STAT6 signaling has been reported to induce TTP in mast cells, which then reduces the expression of TNF-alpha.	bind
18622	4	6611	6	13	NULL	NULL	NULL	statement 1	Process		destabilize					mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_17_2631_s_32	15492321	13 TTP binds to the AU-rich element in the 3' untranslated region of TNF-alpha mRNA to destabilize the mRNA. STAT6 signaling has been reported to induce TTP in mast cells, which then reduces the expression of TNF-alpha.	bind
21045	1	6612	5	13	NULL	NULL	NULL	CXCL1	GP	murine	is					 KC	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
21046	2	6612	5	13	NULL	NULL	NULL	CXCL1	GP	murine	mediate					cell adhesion	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
21047	3	6612	5	13	NULL	NULL	NULL	statement 2	Process		occurs through					CXCR2 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
21051	4	6612	5	13	NULL	NULL	NULL	CX3CL1	GP		induces					cell adhesion	Process	firm			NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
21052	5	6612	5	13	NULL	NULL	NULL	chemokine	GP		bind		directly			CX3CR1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
21053	6	6612	5	13	NULL	NULL	NULL	statement 5	Process		mediates		uniquely			statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
21054	7	6612	5	13	NULL	NULL	NULL	statement 4	Process		does not require					integrins	GP	upregulation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
21055	8	6612	5	13	NULL	NULL	NULL	statement 4	Process		does not require					integrins	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
21056	9	6612	5	13	NULL	NULL	NULL	CX3CL1	GP		mediate					leukocyte trafficking	Process	novel pathway for			NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
21057	10	6612	5	13	NULL	NULL	NULL	CX3CR1	GP		mediate					leukocyte trafficking	Process	novel pathway for			NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
21058	11	6612	5	13	NULL	NULL	NULL	statement 7	Process		suggests					statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
21059	12	6612	5	13	NULL	NULL	NULL	statement 7	Process		suggests					statement 10	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
21060	13	6612	5	13	NULL	NULL	NULL	statement 8	Process		suggests					statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
21061	14	6612	5	13	NULL	NULL	NULL	statement 8	Process		suggests					statement 10	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
56132	15	6612	5	13	NULL	NULL	NULL	KC	GP		is a type of					chemokine	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
18665	1	6612	6	13	NULL	NULL	NULL	KC	GP		bind		directly			CX3CR1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
18666	2	6612	6	13	NULL	NULL	NULL	CX3CL1	GP		mediate					leukocyte trafficking	Process	novel pathway for 			NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
18667	3	6612	6	13	NULL	NULL	NULL	CX3CR1	GP		mediate					 leukocyte trafficking	Process	novel pathway for			NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
18668	4	6612	6	13	NULL	NULL	NULL	KC	GP		mediates					cell adhesion	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
18669	5	6612	6	13	NULL	NULL	NULL	statement 4	Process		occurs through					CXCR2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
18670	6	6612	6	13	NULL	NULL	NULL	CX3CL1	GP		induces					cell adhesion	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
18742	7	6612	6	13	NULL	NULL	NULL	KC	GP		is					murine CXCL1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
18743	8	6612	6	13	NULL	NULL	NULL	CXCR2 	GP		is					receptor for chemokine KC	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
18744	9	6612	6	13	NULL	NULL	NULL	statement 2	Process		occurs simultaneously with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
30312	10	6612	6	13	NULL	NULL	NULL	statement 1	Process		mediates					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
30313	11	6612	6	13	NULL	NULL	NULL	statement 10	Process		does not require					integrin	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
30314	12	6612	6	13	NULL	NULL	NULL	statement 10	Process		does not require					integrins	GP	upregulation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
56133	13	6612	6	13	NULL	NULL	NULL	KC	GP		is a type of					chemokine	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
56134	14	6612	6	13	NULL	NULL	NULL	statement 11	Process		suggest					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
56135	15	6612	6	13	NULL	NULL	NULL	statement 11	Process		suggest					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
56138	16	6612	6	13	NULL	NULL	NULL	statement 12	Process		suggest					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
56139	17	6612	6	13	NULL	NULL	NULL	statement 12	Process		suggest					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_7_1009_s_25	12600915	13, 14 In contrast to cell adhesion mediated by the chemokine KC (murine CXCL1) through its receptor CXCR2, the CX3CL1-induced firm adhesion is uniquely mediated by direct binding of the chemokine to CX3CR1 and does not require the upregulation and activation of integrins, suggesting that CX3CL1 and CX3CR1 mediate a novel pathway for leukocyte trafficking.	bind
20909	1	6613	5	13	NULL	NULL	NULL	CD30	GP		bind					TRAF1	GP		C-terminal region		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2029_s_21	10595933	13, 14 We and other investigators have demonstrated that CD30 binds to tumor necrosis factor receptor-associated factor (TRAF) proteins TRAF1, 2, and 5 in the C-terminal region.	bind
20910	2	6613	5	13	NULL	NULL	NULL	TRAF1	GP		is					tumor necrosis factor receptor-associated factor 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2029_s_21	10595933	13, 14 We and other investigators have demonstrated that CD30 binds to tumor necrosis factor receptor-associated factor (TRAF) proteins TRAF1, 2, and 5 in the C-terminal region.	bind
21062	3	6613	5	13	NULL	NULL	NULL	CD30	GP		bind					TRAF2	GP		C-terminal region		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2029_s_21	10595933	13, 14 We and other investigators have demonstrated that CD30 binds to tumor necrosis factor receptor-associated factor (TRAF) proteins TRAF1, 2, and 5 in the C-terminal region.	bind
21063	4	6613	5	13	NULL	NULL	NULL	TRAF2	GP		is					tumor necrosis factor receptor-associated factor 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2029_s_21	10595933	13, 14 We and other investigators have demonstrated that CD30 binds to tumor necrosis factor receptor-associated factor (TRAF) proteins TRAF1, 2, and 5 in the C-terminal region.	bind
21064	5	6613	5	13	NULL	NULL	NULL	CD30	GP		bind					TRAF5	GP		C-terminal region		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2029_s_21	10595933	13, 14 We and other investigators have demonstrated that CD30 binds to tumor necrosis factor receptor-associated factor (TRAF) proteins TRAF1, 2, and 5 in the C-terminal region.	bind
21065	6	6613	5	13	NULL	NULL	NULL	TRAF5	GP		is					tumor necrosis factor receptor-associated factor 5	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2029_s_21	10595933	13, 14 We and other investigators have demonstrated that CD30 binds to tumor necrosis factor receptor-associated factor (TRAF) proteins TRAF1, 2, and 5 in the C-terminal region.	bind
18623	1	6613	6	13	NULL	NULL	NULL	CD30	GP		bind					TRAF1	GP		C-terminal		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2029_s_21	10595933	13, 14 We and other investigators have demonstrated that CD30 binds to tumor necrosis factor receptor-associated factor (TRAF) proteins TRAF1, 2, and 5 in the C-terminal region.	bind
18624	2	6613	6	13	NULL	NULL	NULL	CD30	GP		bind					TRAF2	GP		C-terminal		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2029_s_21	10595933	13, 14 We and other investigators have demonstrated that CD30 binds to tumor necrosis factor receptor-associated factor (TRAF) proteins TRAF1, 2, and 5 in the C-terminal region.	bind
18625	3	6613	6	13	NULL	NULL	NULL	CD30	GP		bind					TRAF5	GP		C-terminal		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2029_s_21	10595933	13, 14 We and other investigators have demonstrated that CD30 binds to tumor necrosis factor receptor-associated factor (TRAF) proteins TRAF1, 2, and 5 in the C-terminal region.	bind
18626	4	6613	6	13	NULL	NULL	NULL	TRAF1	GP		is					tumor necrosis factor receptor-associated factor1	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2029_s_21	10595933	13, 14 We and other investigators have demonstrated that CD30 binds to tumor necrosis factor receptor-associated factor (TRAF) proteins TRAF1, 2, and 5 in the C-terminal region.	bind
30279	5	6613	6	13	NULL	NULL	NULL	TRAF2	GP		is					tumor necrosis factor receptor-associated factor 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2029_s_21	10595933	13, 14 We and other investigators have demonstrated that CD30 binds to tumor necrosis factor receptor-associated factor (TRAF) proteins TRAF1, 2, and 5 in the C-terminal region.	bind
30280	6	6613	6	13	NULL	NULL	NULL	TRAF5	GP		is					tumor necrosis factor receptor-associated factor 5	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2029_s_21	10595933	13, 14 We and other investigators have demonstrated that CD30 binds to tumor necrosis factor receptor-associated factor (TRAF) proteins TRAF1, 2, and 5 in the C-terminal region.	bind
21112	1	6614	5	13	NULL	NULL	NULL	CD36	GP		is a type of					class B scavenger receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_98_s_34	14563650	13,14  In further support of this hypothesis, CD36 (a class B scavenger receptor that binds both native and modified LDL) is expressed in endothelial cells, has been localized to caveolae, and interacts with Cav-1.	bind
21113	2	6614	5	13	NULL	NULL	NULL	CD36	GP		bind					LDL	GP	native			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_98_s_34	14563650	13,14  In further support of this hypothesis, CD36 (a class B scavenger receptor that binds both native and modified LDL) is expressed in endothelial cells, has been localized to caveolae, and interacts with Cav-1.	bind
21114	3	6614	5	13	NULL	NULL	NULL	CD36	GP		bind					LDL	GP	modified			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_98_s_34	14563650	13,14  In further support of this hypothesis, CD36 (a class B scavenger receptor that binds both native and modified LDL) is expressed in endothelial cells, has been localized to caveolae, and interacts with Cav-1.	bind
21115	4	6614	5	13	NULL	NULL	NULL	CD36	GP		is expressed in					endothelial cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_98_s_34	14563650	13,14  In further support of this hypothesis, CD36 (a class B scavenger receptor that binds both native and modified LDL) is expressed in endothelial cells, has been localized to caveolae, and interacts with Cav-1.	bind
21116	5	6614	5	13	NULL	NULL	NULL	CD36	GP		is localized to					caveolae	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_98_s_34	14563650	13,14  In further support of this hypothesis, CD36 (a class B scavenger receptor that binds both native and modified LDL) is expressed in endothelial cells, has been localized to caveolae, and interacts with Cav-1.	bind
21117	6	6614	5	13	NULL	NULL	NULL	CD36	GP		interacts with					Cav-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_98_s_34	14563650	13,14  In further support of this hypothesis, CD36 (a class B scavenger receptor that binds both native and modified LDL) is expressed in endothelial cells, has been localized to caveolae, and interacts with Cav-1.	bind
18627	1	6614	6	13	NULL	NULL	NULL	CD36	GP		is a type of					a class B scavenger receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_98_s_34	14563650	13,14  In further support of this hypothesis, CD36 (a class B scavenger receptor that binds both native and modified LDL) is expressed in endothelial cells, has been localized to caveolae, and interacts with Cav-1.	bind
18628	2	6614	6	13	NULL	NULL	NULL	CD36	GP		bind					LDL	GP	native			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_98_s_34	14563650	13,14  In further support of this hypothesis, CD36 (a class B scavenger receptor that binds both native and modified LDL) is expressed in endothelial cells, has been localized to caveolae, and interacts with Cav-1.	bind
18629	3	6614	6	13	NULL	NULL	NULL	CD36	GP		bind					LDL	GP	modified			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_98_s_34	14563650	13,14  In further support of this hypothesis, CD36 (a class B scavenger receptor that binds both native and modified LDL) is expressed in endothelial cells, has been localized to caveolae, and interacts with Cav-1.	bind
18630	4	6614	6	13	NULL	NULL	NULL	CD36	GP		is expressed in					endothelial cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_98_s_34	14563650	13,14  In further support of this hypothesis, CD36 (a class B scavenger receptor that binds both native and modified LDL) is expressed in endothelial cells, has been localized to caveolae, and interacts with Cav-1.	bind
18631	5	6614	6	13	NULL	NULL	NULL	CD36	GP		has been localized to					caveolae	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_98_s_34	14563650	13,14  In further support of this hypothesis, CD36 (a class B scavenger receptor that binds both native and modified LDL) is expressed in endothelial cells, has been localized to caveolae, and interacts with Cav-1.	bind
18632	6	6614	6	13	NULL	NULL	NULL	CD36	GP		interacts with					Cav-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_98_s_34	14563650	13,14  In further support of this hypothesis, CD36 (a class B scavenger receptor that binds both native and modified LDL) is expressed in endothelial cells, has been localized to caveolae, and interacts with Cav-1.	bind
21118	1	6615	5	13	NULL	NULL	NULL	Rb	GP		bind					E2F1	GP				NULL	in nonproliferating cells	NULL	NULL	NULL	NULL	gw70_circulationres_93_10_932_s_25	14576193	13,14  In nonproliferating cells, Rb is bound to E2F1 and suppresses its transcriptional activity.	bind
21119	2	6615	5	13	NULL	NULL	NULL	Rb	GP		suppresses					E2F1	GP	transcriptional activity of			NULL	in nonproliferating cells	NULL	NULL	NULL	NULL	gw70_circulationres_93_10_932_s_25	14576193	13,14  In nonproliferating cells, Rb is bound to E2F1 and suppresses its transcriptional activity.	bind
18633	1	6615	6	13	NULL	NULL	NULL	Rb	GP		bind					E2F1	GP				NULL	nonproliferating cells	NULL	NULL	NULL	NULL	gw70_circulationres_93_10_932_s_25	14576193	13,14  In nonproliferating cells, Rb is bound to E2F1 and suppresses its transcriptional activity.	bind
18634	2	6615	6	13	NULL	NULL	NULL	Rb	GP		suppresses					E2F1	GP	transcriptional activity of			NULL	nonproliferating cells	NULL	NULL	NULL	NULL	gw70_circulationres_93_10_932_s_25	14576193	13,14  In nonproliferating cells, Rb is bound to E2F1 and suppresses its transcriptional activity.	bind
21120	1	6616	5	13	NULL	NULL	NULL	Grb2	GP		promotes					ras	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_6_718_s_32	15289381	13,14,19,20    Grb2 promotes the activation of ras via its interaction with the guanine nucleotide exchange factor SOS. 20,21  Finally, pressure overload may lead to the local release of growth factors that bind to cell surface receptor tyrosine kinases, which activate the ras cascade via Grb2 and SOS. 22	bind
21121	2	6616	5	13	NULL	NULL	NULL	Grb2	GP		interacts with					SOS	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_6_718_s_32	15289381	13,14,19,20    Grb2 promotes the activation of ras via its interaction with the guanine nucleotide exchange factor SOS. 20,21  Finally, pressure overload may lead to the local release of growth factors that bind to cell surface receptor tyrosine kinases, which activate the ras cascade via Grb2 and SOS. 22	bind
21122	3	6616	5	13	NULL	NULL	NULL	statement 1	Process		occurs via					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_6_718_s_32	15289381	13,14,19,20    Grb2 promotes the activation of ras via its interaction with the guanine nucleotide exchange factor SOS. 20,21  Finally, pressure overload may lead to the local release of growth factors that bind to cell surface receptor tyrosine kinases, which activate the ras cascade via Grb2 and SOS. 22	bind
21123	4	6616	5	13	NULL	NULL	NULL	pressure overload	ResearchActivity		lead to		may			growth factors	GP	local release of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_6_718_s_32	15289381	13,14,19,20    Grb2 promotes the activation of ras via its interaction with the guanine nucleotide exchange factor SOS. 20,21  Finally, pressure overload may lead to the local release of growth factors that bind to cell surface receptor tyrosine kinases, which activate the ras cascade via Grb2 and SOS. 22	bind
21124	5	6616	5	13	NULL	NULL	NULL	growth factors	GP		bind					receptor tyrosine kinases	GP	cell surface			NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_6_718_s_32	15289381	13,14,19,20    Grb2 promotes the activation of ras via its interaction with the guanine nucleotide exchange factor SOS. 20,21  Finally, pressure overload may lead to the local release of growth factors that bind to cell surface receptor tyrosine kinases, which activate the ras cascade via Grb2 and SOS. 22	bind
21125	6	6616	5	13	NULL	NULL	NULL	receptor tyrosine kinases	GP	cell surface	activate					ras cascade	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_6_718_s_32	15289381	13,14,19,20    Grb2 promotes the activation of ras via its interaction with the guanine nucleotide exchange factor SOS. 20,21  Finally, pressure overload may lead to the local release of growth factors that bind to cell surface receptor tyrosine kinases, which activate the ras cascade via Grb2 and SOS. 22	bind
21126	7	6616	5	13	NULL	NULL	NULL	statement 6	Process		occurs via					Grb2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_6_718_s_32	15289381	13,14,19,20    Grb2 promotes the activation of ras via its interaction with the guanine nucleotide exchange factor SOS. 20,21  Finally, pressure overload may lead to the local release of growth factors that bind to cell surface receptor tyrosine kinases, which activate the ras cascade via Grb2 and SOS. 22	bind
21127	8	6616	5	13	NULL	NULL	NULL	statement 6	Process		occurs via					SOS	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_6_718_s_32	15289381	13,14,19,20    Grb2 promotes the activation of ras via its interaction with the guanine nucleotide exchange factor SOS. 20,21  Finally, pressure overload may lead to the local release of growth factors that bind to cell surface receptor tyrosine kinases, which activate the ras cascade via Grb2 and SOS. 22	bind
56176	9	6616	5	13	NULL	NULL	NULL	SOS	GP		is a type of					guanine nucleotide exchange factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_6_718_s_32	15289381	13,14,19,20    Grb2 promotes the activation of ras via its interaction with the guanine nucleotide exchange factor SOS. 20,21  Finally, pressure overload may lead to the local release of growth factors that bind to cell surface receptor tyrosine kinases, which activate the ras cascade via Grb2 and SOS. 22	bind
18635	1	6616	6	13	NULL	NULL	NULL	Grb2	GP		interacts with					SOS	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_6_718_s_32	15289381	13,14,19,20    Grb2 promotes the activation of ras via its interaction with the guanine nucleotide exchange factor SOS. 20,21  Finally, pressure overload may lead to the local release of growth factors that bind to cell surface receptor tyrosine kinases, which activate the ras cascade via Grb2 and SOS. 22	bind
18636	2	6616	6	13	NULL	NULL	NULL	Grb2	GP		promotes					Ras	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_6_718_s_32	15289381	13,14,19,20    Grb2 promotes the activation of ras via its interaction with the guanine nucleotide exchange factor SOS. 20,21  Finally, pressure overload may lead to the local release of growth factors that bind to cell surface receptor tyrosine kinases, which activate the ras cascade via Grb2 and SOS. 22	bind
18637	3	6616	6	13	NULL	NULL	NULL	statement 1	Process		occurs via					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_6_718_s_32	15289381	13,14,19,20    Grb2 promotes the activation of ras via its interaction with the guanine nucleotide exchange factor SOS. 20,21  Finally, pressure overload may lead to the local release of growth factors that bind to cell surface receptor tyrosine kinases, which activate the ras cascade via Grb2 and SOS. 22	bind
18638	4	6616	6	13	NULL	NULL	NULL	SOS	GP		is a type of					guanine nucleotide exchange factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_6_718_s_32	15289381	13,14,19,20    Grb2 promotes the activation of ras via its interaction with the guanine nucleotide exchange factor SOS. 20,21  Finally, pressure overload may lead to the local release of growth factors that bind to cell surface receptor tyrosine kinases, which activate the ras cascade via Grb2 and SOS. 22	bind
18639	5	6616	6	13	NULL	NULL	NULL	growth factor	GP		bind					 receptor tyrosine kinases	GP	cell surface			NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_6_718_s_32	15289381	13,14,19,20    Grb2 promotes the activation of ras via its interaction with the guanine nucleotide exchange factor SOS. 20,21  Finally, pressure overload may lead to the local release of growth factors that bind to cell surface receptor tyrosine kinases, which activate the ras cascade via Grb2 and SOS. 22	bind
18640	6	6616	6	13	NULL	NULL	NULL	pressure overload	ResearchActivity		may lead to					growth factor	GP	release of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_6_718_s_32	15289381	13,14,19,20    Grb2 promotes the activation of ras via its interaction with the guanine nucleotide exchange factor SOS. 20,21  Finally, pressure overload may lead to the local release of growth factors that bind to cell surface receptor tyrosine kinases, which activate the ras cascade via Grb2 and SOS. 22	bind
18641	7	6616	6	13	NULL	NULL	NULL	 receptor tyrosine kinases	GP	cell surface	activate					ras cascade	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_6_718_s_32	15289381	13,14,19,20    Grb2 promotes the activation of ras via its interaction with the guanine nucleotide exchange factor SOS. 20,21  Finally, pressure overload may lead to the local release of growth factors that bind to cell surface receptor tyrosine kinases, which activate the ras cascade via Grb2 and SOS. 22	bind
18642	8	6616	6	13	NULL	NULL	NULL	statement 7	Process		occurs via					Grb2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_6_718_s_32	15289381	13,14,19,20    Grb2 promotes the activation of ras via its interaction with the guanine nucleotide exchange factor SOS. 20,21  Finally, pressure overload may lead to the local release of growth factors that bind to cell surface receptor tyrosine kinases, which activate the ras cascade via Grb2 and SOS. 22	bind
18643	9	6616	6	13	NULL	NULL	NULL	statement 7	Process		occurs via					SOS	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_6_718_s_32	15289381	13,14,19,20    Grb2 promotes the activation of ras via its interaction with the guanine nucleotide exchange factor SOS. 20,21  Finally, pressure overload may lead to the local release of growth factors that bind to cell surface receptor tyrosine kinases, which activate the ras cascade via Grb2 and SOS. 22	bind
21144	1	6617	5	13	NULL	NULL	NULL	VEGF	GP		mediate					chemotaxis	Process	endothelial			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_12_1257_s_157	15920019	13,18,31   As has been previously reported, stable coexpression of Npn-1 and VEGFR2 enhanced VEGF-mediated endothelial chemotaxis, 19,43  and Npn-1 inhibition partially attenuated human pulmonary artery VEGF-mediated endothelial cell migration.	bind
21145	2	6617	5	13	NULL	NULL	NULL	Npn-1	GP		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_12_1257_s_157	15920019	13,18,31   As has been previously reported, stable coexpression of Npn-1 and VEGFR2 enhanced VEGF-mediated endothelial chemotaxis, 19,43  and Npn-1 inhibition partially attenuated human pulmonary artery VEGF-mediated endothelial cell migration.	bind
21146	5	6617	5	13	NULL	NULL	NULL	VEGF	GP		mediate					cell migration	Process	endothelial			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_12_1257_s_157	15920019	13,18,31   As has been previously reported, stable coexpression of Npn-1 and VEGFR2 enhanced VEGF-mediated endothelial chemotaxis, 19,43  and Npn-1 inhibition partially attenuated human pulmonary artery VEGF-mediated endothelial cell migration.	bind
21147	6	6617	5	13	NULL	NULL	NULL	Npn-1	GP	inhibition	attenuates		partially			statement 3	Process				NULL	human pulmonary artery	NULL	NULL	NULL	NULL	gw70_circulationres_96_12_1257_s_157	15920019	13,18,31   As has been previously reported, stable coexpression of Npn-1 and VEGFR2 enhanced VEGF-mediated endothelial chemotaxis, 19,43  and Npn-1 inhibition partially attenuated human pulmonary artery VEGF-mediated endothelial cell migration.	bind
56177	3	6617	5	13	NULL	NULL	NULL	VEGFR2	GP		enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_12_1257_s_157	15920019	13,18,31   As has been previously reported, stable coexpression of Npn-1 and VEGFR2 enhanced VEGF-mediated endothelial chemotaxis, 19,43  and Npn-1 inhibition partially attenuated human pulmonary artery VEGF-mediated endothelial cell migration.	bind
56178	4	6617	5	13	NULL	NULL	NULL	statement 2	Process		occur simultaneous with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_12_1257_s_157	15920019	13,18,31   As has been previously reported, stable coexpression of Npn-1 and VEGFR2 enhanced VEGF-mediated endothelial chemotaxis, 19,43  and Npn-1 inhibition partially attenuated human pulmonary artery VEGF-mediated endothelial cell migration.	bind
18644	1	6617	6	13	NULL	NULL	NULL	VEGF	GP		mediates					 chemotaxis	Process	endothelial			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_12_1257_s_157	15920019	13,18,31   As has been previously reported, stable coexpression of Npn-1 and VEGFR2 enhanced VEGF-mediated endothelial chemotaxis, 19,43  and Npn-1 inhibition partially attenuated human pulmonary artery VEGF-mediated endothelial cell migration.	bind
18645	2	6617	6	13	NULL	NULL	NULL	Npn-1	GP		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_12_1257_s_157	15920019	13,18,31   As has been previously reported, stable coexpression of Npn-1 and VEGFR2 enhanced VEGF-mediated endothelial chemotaxis, 19,43  and Npn-1 inhibition partially attenuated human pulmonary artery VEGF-mediated endothelial cell migration.	bind
18646	3	6617	6	13	NULL	NULL	NULL	VEGFR2	GP		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_12_1257_s_157	15920019	13,18,31   As has been previously reported, stable coexpression of Npn-1 and VEGFR2 enhanced VEGF-mediated endothelial chemotaxis, 19,43  and Npn-1 inhibition partially attenuated human pulmonary artery VEGF-mediated endothelial cell migration.	bind
18647	4	6617	6	13	NULL	NULL	NULL	statement 2	Process		occurs simultaneously with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_12_1257_s_157	15920019	13,18,31   As has been previously reported, stable coexpression of Npn-1 and VEGFR2 enhanced VEGF-mediated endothelial chemotaxis, 19,43  and Npn-1 inhibition partially attenuated human pulmonary artery VEGF-mediated endothelial cell migration.	bind
18648	6	6617	6	13	NULL	NULL	NULL	Npn-1	GP	inhibition of	attenuates		partially			statement 5	Process				NULL	human pulmonary artery	NULL	NULL	NULL	NULL	gw70_circulationres_96_12_1257_s_157	15920019	13,18,31   As has been previously reported, stable coexpression of Npn-1 and VEGFR2 enhanced VEGF-mediated endothelial chemotaxis, 19,43  and Npn-1 inhibition partially attenuated human pulmonary artery VEGF-mediated endothelial cell migration.	bind
56180	5	6617	6	13	NULL	NULL	NULL	VEGF	GP		mediate					cell migration	Process	endothelial			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_12_1257_s_157	15920019	13,18,31   As has been previously reported, stable coexpression of Npn-1 and VEGFR2 enhanced VEGF-mediated endothelial chemotaxis, 19,43  and Npn-1 inhibition partially attenuated human pulmonary artery VEGF-mediated endothelial cell migration.	bind
21148	1	6618	5	13	NULL	NULL	NULL				is phosphorylated by		constitutively	Thr495		PKCs	GP				NULL	in endothelial cells	NULL	NULL	NULL	NULL	gw70_circulation_109_3_399_s_140	14707024	13,29,30   By contrast, Thr495 is constitutively phosphorylated by PKCs in the endothelial cells investigated to date, and it is a negative regulatory site, ie, phosphorylation causes a decrease in enzyme activity through interference with the binding of calmodulin to the calmodulin-binding domain.	bind
21150	2	6618	5	13	NULL	NULL	NULL	calmodulin	GP		bind								calmodulin-binding domain		NULL		NULL	NULL	NULL	NULL	gw70_circulation_109_3_399_s_140	14707024	13,29,30   By contrast, Thr495 is constitutively phosphorylated by PKCs in the endothelial cells investigated to date, and it is a negative regulatory site, ie, phosphorylation causes a decrease in enzyme activity through interference with the binding of calmodulin to the calmodulin-binding domain.	bind
18649	1	6618	6	13	NULL	NULL	NULL				is phosphorylated 		constitutively	Thr495		PKC	GP				NULL	endothelial cells	NULL	NULL	NULL	NULL	gw70_circulation_109_3_399_s_140	14707024	13,29,30   By contrast, Thr495 is constitutively phosphorylated by PKCs in the endothelial cells investigated to date, and it is a negative regulatory site, ie, phosphorylation causes a decrease in enzyme activity through interference with the binding of calmodulin to the calmodulin-binding domain.	bind
18650	2	6618	6	13	NULL	NULL	NULL	calmodulin	GP		bind								calmodulin-binding domain		NULL		NULL	NULL	NULL	NULL	gw70_circulation_109_3_399_s_140	14707024	13,29,30   By contrast, Thr495 is constitutively phosphorylated by PKCs in the endothelial cells investigated to date, and it is a negative regulatory site, ie, phosphorylation causes a decrease in enzyme activity through interference with the binding of calmodulin to the calmodulin-binding domain.	bind
21152	1	6619	5	13	NULL	NULL	NULL	13- cis-RA	Chemical		does not bind					retinoic acid receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_35008_s_245	9857033	13- cis-RA does not bind to retinoic acid receptors and is thought to act through its metabolites including ATRA ( 3).	bind
21153	2	6619	5	13	NULL	NULL	NULL	13-cis-RA	Chemical		act through		might			ATRA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_35008_s_245	9857033	13- cis-RA does not bind to retinoic acid receptors and is thought to act through its metabolites including ATRA ( 3).	bind
21154	3	6619	5	13	NULL	NULL	NULL	ATRA	Chemical		is a metabolite of					13- cis-RA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_35008_s_245	9857033	13- cis-RA does not bind to retinoic acid receptors and is thought to act through its metabolites including ATRA ( 3).	bind
18651	1	6619	6	13	NULL	NULL	NULL	13- cis-RA	Chemical		does not bind					retinoic acid receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_35008_s_245	9857033	13- cis-RA does not bind to retinoic acid receptors and is thought to act through its metabolites including ATRA ( 3).	bind
56182	3	6619	6	13	NULL	NULL	NULL	ATRA	Chemical		is a metabolite of					13- cis-RA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_35008_s_245	9857033	13- cis-RA does not bind to retinoic acid receptors and is thought to act through its metabolites including ATRA ( 3).	bind
56183	2	6619	6	13	NULL	NULL	NULL	13- cis-RA	Chemical		act through		might			ATRA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_35008_s_245	9857033	13- cis-RA does not bind to retinoic acid receptors and is thought to act through its metabolites including ATRA ( 3).	bind
21155	2	6620	5	13	NULL	NULL	NULL	statement 1	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_7988_s_8	14662773	13-Mers containing these profilin-like segments bound actin in fluorescent anisotropy studies and competed with profilin for binding to actin.	bind
21156	3	6620	5	13	NULL	NULL	NULL	profilin	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_7988_s_8	14662773	13-Mers containing these profilin-like segments bound actin in fluorescent anisotropy studies and competed with profilin for binding to actin.	bind
21157	4	6620	5	13	NULL	NULL	NULL	statement 2	Process		competes with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_7988_s_8	14662773	13-Mers containing these profilin-like segments bound actin in fluorescent anisotropy studies and competed with profilin for binding to actin.	bind
44667	1	6620	5	13	NULL	NULL	NULL	13-Mers	GP		contain					profilin-like segments	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_7988_s_8	14662773	13-Mers containing these profilin-like segments bound actin in fluorescent anisotropy studies and competed with profilin for binding to actin.	bind
18652	1	6620	6	13	NULL	NULL	NULL	profilin	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_7988_s_8	14662773	13-Mers containing these profilin-like segments bound actin in fluorescent anisotropy studies and competed with profilin for binding to actin.	bind
18653	2	6620	6	13	NULL	NULL	NULL	13-Mers	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_7988_s_8	14662773	13-Mers containing these profilin-like segments bound actin in fluorescent anisotropy studies and competed with profilin for binding to actin.	bind
18654	3	6620	6	13	NULL	NULL	NULL	statement 1	Process		competes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_7988_s_8	14662773	13-Mers containing these profilin-like segments bound actin in fluorescent anisotropy studies and competed with profilin for binding to actin.	bind
56184	4	6620	6	13	NULL	NULL	NULL	13-Mers	GP		contain					profilin-like segments	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_7988_s_8	14662773	13-Mers containing these profilin-like segments bound actin in fluorescent anisotropy studies and competed with profilin for binding to actin.	bind
21158	1	6621	5	13	NULL	NULL	NULL	CsA	Chemical	prophylactic administration of 	inhibit					cardiac hypertrophy	Process	development of			NULL	rat	NULL	NULL	NULL	NULL	gw60_circulationres_84_6_633_s_234	10189351	139  In addition, prophylactic administration of CsA inhibited the development of cardiac hypertrophy after suprarenal banding of the abdominal aorta in the rat.	bind
21159	2	6621	5	13	NULL	NULL	NULL	statement 1	Process		occurs after					 abdominal aorta	OrganismPart	suprarenal banding of			NULL	rat	NULL	NULL	NULL	NULL	gw60_circulationres_84_6_633_s_234	10189351	139  In addition, prophylactic administration of CsA inhibited the development of cardiac hypertrophy after suprarenal banding of the abdominal aorta in the rat.	bind
18655	1	6621	6	13	NULL	NULL	NULL	CsA	Chemical		inhibits					cardiac hypertrophy	Process	development of 			NULL	rat	NULL	NULL	NULL	NULL	gw60_circulationres_84_6_633_s_234	10189351	139  In addition, prophylactic administration of CsA inhibited the development of cardiac hypertrophy after suprarenal banding of the abdominal aorta in the rat.	bind
30278	2	6621	6	13	NULL	NULL	NULL	statement 1	Process		occurs after					abdominal aorta	OrganismPart	suprarenal banding of			NULL	rat	NULL	NULL	NULL	NULL	gw60_circulationres_84_6_633_s_234	10189351	139  In addition, prophylactic administration of CsA inhibited the development of cardiac hypertrophy after suprarenal banding of the abdominal aorta in the rat.	bind
21372	1	6622	5	13	NULL	NULL	NULL	SCP-2	GP		interacts with					fatty acid	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_50_35425_s_125	10585412	13C Chemical Shifts of SCP-2 Bound Versus Unbound Fully Enriched [1318]Oleate-- Prior to using 13C-labeled fatty acids to determine if the cholesterol and fatty acid binding sites were the same or different, it was necessary to first characterize the interaction of fatty acid with SCP-2.	bind
18656	1	6622	6	13	NULL	NULL	NULL	fatty acid	Chemical		interacts with					SCP-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_50_35425_s_125	10585412	13C Chemical Shifts of SCP-2 Bound Versus Unbound Fully Enriched [1318]Oleate-- Prior to using 13C-labeled fatty acids to determine if the cholesterol and fatty acid binding sites were the same or different, it was necessary to first characterize the interaction of fatty acid with SCP-2.	bind
21373	1	6623	5	13	NULL	NULL	NULL	palmitate	Chemical		bind					HSA	GP		domain III		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_50_17958_s_130	16330771	13C NMR spectra were obtained to study [13]palmitate binding to domain III of HSA.	bind
18657	1	6623	6	13	NULL	NULL	NULL	palmitate	Chemical		bind					HSA	GP		domain III		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_50_17958_s_130	16330771	13C NMR spectra were obtained to study [13]palmitate binding to domain III of HSA.	bind
21374	1	6624	5	13	NULL	NULL	NULL	XPA	GP		bind					RPA	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2635_s_271	11410673	14       Matsuda,T., Saijo,M., Kuraoka,I., Kobayashi,T., Nakatsu,Y., Nagai,A., Enjoji,T., Masutani,C., Sugasawa,K., Hanoaka,F. et al. (1995) DNA repair protein XPA binds replication protein A (RPA).	bind
21375	2	6624	5	13	NULL	NULL	NULL	RPA	GP		is					replication protein A	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2635_s_271	11410673	14       Matsuda,T., Saijo,M., Kuraoka,I., Kobayashi,T., Nakatsu,Y., Nagai,A., Enjoji,T., Masutani,C., Sugasawa,K., Hanoaka,F. et al. (1995) DNA repair protein XPA binds replication protein A (RPA).	bind
30310	3	6624	5	13	NULL	NULL	NULL	XPA	GP		is a type of					DNA repair protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2635_s_271	11410673	14       Matsuda,T., Saijo,M., Kuraoka,I., Kobayashi,T., Nakatsu,Y., Nagai,A., Enjoji,T., Masutani,C., Sugasawa,K., Hanoaka,F. et al. (1995) DNA repair protein XPA binds replication protein A (RPA).	bind
18658	1	6624	6	13	NULL	NULL	NULL	XPA	GP		bind					RPA	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2635_s_271	11410673	14       Matsuda,T., Saijo,M., Kuraoka,I., Kobayashi,T., Nakatsu,Y., Nagai,A., Enjoji,T., Masutani,C., Sugasawa,K., Hanoaka,F. et al. (1995) DNA repair protein XPA binds replication protein A (RPA).	bind
18659	2	6624	6	13	NULL	NULL	NULL	XPA	GP		is a type of					DNA repair protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2635_s_271	11410673	14       Matsuda,T., Saijo,M., Kuraoka,I., Kobayashi,T., Nakatsu,Y., Nagai,A., Enjoji,T., Masutani,C., Sugasawa,K., Hanoaka,F. et al. (1995) DNA repair protein XPA binds replication protein A (RPA).	bind
18660	3	6624	6	13	NULL	NULL	NULL	RPA	GP		is					replication protein A	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2635_s_271	11410673	14       Matsuda,T., Saijo,M., Kuraoka,I., Kobayashi,T., Nakatsu,Y., Nagai,A., Enjoji,T., Masutani,C., Sugasawa,K., Hanoaka,F. et al. (1995) DNA repair protein XPA binds replication protein A (RPA).	bind
21377	1	6625	5	13	NULL	NULL	NULL	Rap1p	GP		is					telomere binding protein	GP	yeast			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_11_2382_s_413	11376157	14       Ray,A. and Runge,K.W. (1998) The C-terminus of the major yeast telomere binding protein Rap1p enhances telomere formation.	bind
21378	2	6625	5	13	NULL	NULL	NULL	Rap1p	GP		enhances			C-terminus		telomere	NucleicAcid	formation of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_11_2382_s_413	11376157	14       Ray,A. and Runge,K.W. (1998) The C-terminus of the major yeast telomere binding protein Rap1p enhances telomere formation.	bind
18661	1	6625	6	13	NULL	NULL	NULL	Rap1p	GP		is					telomere binding protein	GP	yeast			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_11_2382_s_413	11376157	14       Ray,A. and Runge,K.W. (1998) The C-terminus of the major yeast telomere binding protein Rap1p enhances telomere formation.	bind
18662	2	6625	6	13	NULL	NULL	NULL	Rap1p	GP		enhances			C-terminus		telomere	NucleicAcid	formation of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_11_2382_s_413	11376157	14       Ray,A. and Runge,K.W. (1998) The C-terminus of the major yeast telomere binding protein Rap1p enhances telomere formation.	bind
21381	1	6626	5	13	NULL	NULL	NULL	Grb2	GP		bind					Fak	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_7_558_s_131	11009560	14  As shown in Figure 7A  , acute pressure overload increased the amount of Grb2 binding to Fak in parallel with activation of the Fak/c-Src complex.	bind
21383	2	6626	5	13	NULL	NULL	NULL	acute pressure overload	ResearchActivity		increases					statement 1	Process	amount of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_7_558_s_131	11009560	14  As shown in Figure 7A  , acute pressure overload increased the amount of Grb2 binding to Fak in parallel with activation of the Fak/c-Src complex.	bind
21385	3	6626	5	13	NULL	NULL	NULL	acute pressure overload	ResearchActivity		increases					Fak/c-Src complex	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_7_558_s_131	11009560	14  As shown in Figure 7A  , acute pressure overload increased the amount of Grb2 binding to Fak in parallel with activation of the Fak/c-Src complex.	bind
21387	4	6626	5	13	NULL	NULL	NULL	statement 2	Process		in parallel with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_7_558_s_131	11009560	14  As shown in Figure 7A  , acute pressure overload increased the amount of Grb2 binding to Fak in parallel with activation of the Fak/c-Src complex.	bind
18671	1	6626	6	13	NULL	NULL	NULL	Grb2	GP		bind					Fak	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_7_558_s_131	11009560	14  As shown in Figure 7A  , acute pressure overload increased the amount of Grb2 binding to Fak in parallel with activation of the Fak/c-Src complex.	bind
18672	2	6626	6	13	NULL	NULL	NULL	acute pressure overload	ResearchActivity		increased					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_7_558_s_131	11009560	14  As shown in Figure 7A  , acute pressure overload increased the amount of Grb2 binding to Fak in parallel with activation of the Fak/c-Src complex.	bind
18673	3	6626	6	13	NULL	NULL	NULL	acute pressure overload	ResearchActivity		increased					FAK/c-Src complex	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_7_558_s_131	11009560	14  As shown in Figure 7A  , acute pressure overload increased the amount of Grb2 binding to Fak in parallel with activation of the Fak/c-Src complex.	bind
30277	4	6626	6	13	NULL	NULL	NULL	statement 2	Process		in parallel with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_7_558_s_131	11009560	14  As shown in Figure 7A  , acute pressure overload increased the amount of Grb2 binding to Fak in parallel with activation of the Fak/c-Src complex.	bind
21391	1	6627	5	13	NULL	NULL	NULL	TRADD	GP		bind			N-terminal portion		TRAF-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_3_997_s_28	10702415	14  he N-terminal portion of TRADD binds the TNF receptor-associated factor 2 (TRAF-2), and other more recently identified proteins such as RIP, ultimately resulting in the activation of NF-kappaB.	bind
21392	2	6627	5	13	NULL	NULL	NULL	TRAF-2	GP		is					TNF receptor-associated factor 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_3_997_s_28	10702415	14  he N-terminal portion of TRADD binds the TNF receptor-associated factor 2 (TRAF-2), and other more recently identified proteins such as RIP, ultimately resulting in the activation of NF-kappaB.	bind
21393	3	6627	5	13	NULL	NULL	NULL	TRADD	GP		bind			N-terminal portion		RIP	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_3_997_s_28	10702415	14  he N-terminal portion of TRADD binds the TNF receptor-associated factor 2 (TRAF-2), and other more recently identified proteins such as RIP, ultimately resulting in the activation of NF-kappaB.	bind
21395	4	6627	5	13	NULL	NULL	NULL	statement 1	Process		results in					NF-kappaB	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_3_997_s_28	10702415	14  he N-terminal portion of TRADD binds the TNF receptor-associated factor 2 (TRAF-2), and other more recently identified proteins such as RIP, ultimately resulting in the activation of NF-kappaB.	bind
21396	5	6627	5	13	NULL	NULL	NULL	statement 3	Process		results in					NF-kappaB	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_3_997_s_28	10702415	14  he N-terminal portion of TRADD binds the TNF receptor-associated factor 2 (TRAF-2), and other more recently identified proteins such as RIP, ultimately resulting in the activation of NF-kappaB.	bind
18674	1	6627	6	13	NULL	NULL	NULL	TRADD	GP		bind			N terminal		TRAF-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_3_997_s_28	10702415	14  he N-terminal portion of TRADD binds the TNF receptor-associated factor 2 (TRAF-2), and other more recently identified proteins such as RIP, ultimately resulting in the activation of NF-kappaB.	bind
18675	2	6627	6	13	NULL	NULL	NULL	TRAF-2	GP		is					TNF receptor-associated factor 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_3_997_s_28	10702415	14  he N-terminal portion of TRADD binds the TNF receptor-associated factor 2 (TRAF-2), and other more recently identified proteins such as RIP, ultimately resulting in the activation of NF-kappaB.	bind
18676	3	6627	6	13	NULL	NULL	NULL	TRADD	GP		bind			N-terminal		RIP	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_3_997_s_28	10702415	14  he N-terminal portion of TRADD binds the TNF receptor-associated factor 2 (TRAF-2), and other more recently identified proteins such as RIP, ultimately resulting in the activation of NF-kappaB.	bind
18677	4	6627	6	13	NULL	NULL	NULL	statement 1	Process		results in					NF-kappaB	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_3_997_s_28	10702415	14  he N-terminal portion of TRADD binds the TNF receptor-associated factor 2 (TRAF-2), and other more recently identified proteins such as RIP, ultimately resulting in the activation of NF-kappaB.	bind
18678	5	6627	6	13	NULL	NULL	NULL	statement 3	Process		results in					NF-kappaB	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_3_997_s_28	10702415	14  he N-terminal portion of TRADD binds the TNF receptor-associated factor 2 (TRAF-2), and other more recently identified proteins such as RIP, ultimately resulting in the activation of NF-kappaB.	bind
21398	2	6628	5	13	NULL	NULL	NULL	sPLA2	GP		bind					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulationres_86_6_610_s_27	10746993	14  Later, they studied the binding of sPLA2 to collagen-associated proteoglycans in vitro and found that sPLA2 binds to the glycosaminoglycan chains of biglycan.	bind
21400	3	6628	5	13	NULL	NULL	NULL	sPLA2	GP		bind					biglycan	GP		glycosaminoglycan chains 		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulationres_86_6_610_s_27	10746993	14  Later, they studied the binding of sPLA2 to collagen-associated proteoglycans in vitro and found that sPLA2 binds to the glycosaminoglycan chains of biglycan.	bind
56200	1	6628	5	13	NULL	NULL	NULL	collagen	GP		associate with					proteoglycans	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_6_610_s_27	10746993	14  Later, they studied the binding of sPLA2 to collagen-associated proteoglycans in vitro and found that sPLA2 binds to the glycosaminoglycan chains of biglycan.	bind
18679	1	6628	6	13	NULL	NULL	NULL	sPLA2	GP		bind					biglycan	GP		glycosaminoglycan chains		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulationres_86_6_610_s_27	10746993	14  Later, they studied the binding of sPLA2 to collagen-associated proteoglycans in vitro and found that sPLA2 binds to the glycosaminoglycan chains of biglycan.	bind
56201	2	6628	6	13	NULL	NULL	NULL	collagen	GP		associate with					proteoglycans	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_6_610_s_27	10746993	14  Later, they studied the binding of sPLA2 to collagen-associated proteoglycans in vitro and found that sPLA2 binds to the glycosaminoglycan chains of biglycan.	bind
56203	3	6628	6	13	NULL	NULL	NULL	sPLA2	GP		bind					statement 2	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulationres_86_6_610_s_27	10746993	14  Later, they studied the binding of sPLA2 to collagen-associated proteoglycans in vitro and found that sPLA2 binds to the glycosaminoglycan chains of biglycan.	bind
21402	1	6629	5	13	NULL	NULL	NULL	 NT	GP		bind					TrkB	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_2_405_s_229	10027399	14  NT also bind to truncated TK- receptors, identified for TrkB and TrkC, 15- 18  which may function as dominant negative isoforms, 20  or immunoadhesins.	bind
21406	2	6629	5	13	NULL	NULL	NULL	NT	GP		bind					TrkC	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_2_405_s_229	10027399	14  NT also bind to truncated TK- receptors, identified for TrkB and TrkC, 15- 18  which may function as dominant negative isoforms, 20  or immunoadhesins.	bind
21409	3	6629	5	13	NULL	NULL	NULL	TrkB	GP		is					truncated TK- receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_2_405_s_229	10027399	14  NT also bind to truncated TK- receptors, identified for TrkB and TrkC, 15- 18  which may function as dominant negative isoforms, 20  or immunoadhesins.	bind
21410	4	6629	5	13	NULL	NULL	NULL	TrkC	GP		is					truncated TK- receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_2_405_s_229	10027399	14  NT also bind to truncated TK- receptors, identified for TrkB and TrkC, 15- 18  which may function as dominant negative isoforms, 20  or immunoadhesins.	bind
21411	5	6629	5	13	NULL	NULL	NULL	TrkB	GP		function as		may			dominant negative isoforms	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_2_405_s_229	10027399	14  NT also bind to truncated TK- receptors, identified for TrkB and TrkC, 15- 18  which may function as dominant negative isoforms, 20  or immunoadhesins.	bind
21412	6	6629	5	13	NULL	NULL	NULL	TrkC	GP		function as		may			dominant negative isoforms	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_2_405_s_229	10027399	14  NT also bind to truncated TK- receptors, identified for TrkB and TrkC, 15- 18  which may function as dominant negative isoforms, 20  or immunoadhesins.	bind
21413	7	6629	5	13	NULL	NULL	NULL	TrkB	GP		function as		may			immunoadhesins	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_2_405_s_229	10027399	14  NT also bind to truncated TK- receptors, identified for TrkB and TrkC, 15- 18  which may function as dominant negative isoforms, 20  or immunoadhesins.	bind
21415	8	6629	5	13	NULL	NULL	NULL	TrkC	GP		function as		may			immunoadhesins	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_2_405_s_229	10027399	14  NT also bind to truncated TK- receptors, identified for TrkB and TrkC, 15- 18  which may function as dominant negative isoforms, 20  or immunoadhesins.	bind
18680	1	6629	6	13	NULL	NULL	NULL	NT	GP		bind					TK-receptors	GP	truncated			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_2_405_s_229	10027399	14  NT also bind to truncated TK- receptors, identified for TrkB and TrkC, 15- 18  which may function as dominant negative isoforms, 20  or immunoadhesins.	bind
21419	1	6630	5	13	NULL	NULL	NULL	macrophages	Cell	human	bind					LDL	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_149_s_208	9012650	14  The GAG-induced alterations are associated with an increase in LDL binding and degradation by human monocyte - derived macrophages and smooth muscle cells.	bind
21422	2	6630	5	13	NULL	NULL	NULL	smooth muscle cells	Cell	human	bind					LDL	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_149_s_208	9012650	14  The GAG-induced alterations are associated with an increase in LDL binding and degradation by human monocyte - derived macrophages and smooth muscle cells.	bind
21425	3	6630	5	13	NULL	NULL	NULL	GAG-induced alterations	Process		is associated with					statement 1	Process	increase in			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_149_s_208	9012650	14  The GAG-induced alterations are associated with an increase in LDL binding and degradation by human monocyte - derived macrophages and smooth muscle cells.	bind
21426	4	6630	5	13	NULL	NULL	NULL	GAG-induced alterations	Process		is associated with					statement 2	Process	increase in			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_149_s_208	9012650	14  The GAG-induced alterations are associated with an increase in LDL binding and degradation by human monocyte - derived macrophages and smooth muscle cells.	bind
21427	5	6630	5	13	NULL	NULL	NULL	macrophages	Cell	human 	degrade					LDL	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_149_s_208	9012650	14  The GAG-induced alterations are associated with an increase in LDL binding and degradation by human monocyte - derived macrophages and smooth muscle cells.	bind
21430	6	6630	5	13	NULL	NULL	NULL	smooth muscle cells	Cell	human	degrade					LDL	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_149_s_208	9012650	14  The GAG-induced alterations are associated with an increase in LDL binding and degradation by human monocyte - derived macrophages and smooth muscle cells.	bind
21431	7	6630	5	13	NULL	NULL	NULL	GAG-induced alterations	Process		is associated with					statement 5	Process	increase in			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_149_s_208	9012650	14  The GAG-induced alterations are associated with an increase in LDL binding and degradation by human monocyte - derived macrophages and smooth muscle cells.	bind
21432	8	6630	5	13	NULL	NULL	NULL	GAG-induced alterations	Process		is associated with					statement 6	Process	increase in			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_149_s_208	9012650	14  The GAG-induced alterations are associated with an increase in LDL binding and degradation by human monocyte - derived macrophages and smooth muscle cells.	bind
56204	9	6630	5	13	NULL	NULL	NULL	macrophages	Cell		derived from					monocyte	Cell	human			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_149_s_208	9012650	14  The GAG-induced alterations are associated with an increase in LDL binding and degradation by human monocyte - derived macrophages and smooth muscle cells.	bind
18912	1	6630	6	13	NULL	NULL	NULL	 macrophages	Cell	human	bind					LDL	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_149_s_208	9012650	14  The GAG-induced alterations are associated with an increase in LDL binding and degradation by human monocyte - derived macrophages and smooth muscle cells.	bind
18913	2	6630	6	13	NULL	NULL	NULL	smooth muscle cells	Cell	human	bind					LDL	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_149_s_208	9012650	14  The GAG-induced alterations are associated with an increase in LDL binding and degradation by human monocyte - derived macrophages and smooth muscle cells.	bind
18942	3	6630	6	13	NULL	NULL	NULL	GAG-induced alterations	Process		increase					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_149_s_208	9012650	14  The GAG-induced alterations are associated with an increase in LDL binding and degradation by human monocyte - derived macrophages and smooth muscle cells.	bind
18943	4	6630	6	13	NULL	NULL	NULL	GAG-induced alterations	Process		increase					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_149_s_208	9012650	14  The GAG-induced alterations are associated with an increase in LDL binding and degradation by human monocyte - derived macrophages and smooth muscle cells.	bind
30315	5	6630	6	13	NULL	NULL	NULL	macrophages	Cell	human	degrade					LDL	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_149_s_208	9012650	14  The GAG-induced alterations are associated with an increase in LDL binding and degradation by human monocyte - derived macrophages and smooth muscle cells.	bind
30316	6	6630	6	13	NULL	NULL	NULL	smooth muscle cells	Cell	human	degrade					LDL	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_149_s_208	9012650	14  The GAG-induced alterations are associated with an increase in LDL binding and degradation by human monocyte - derived macrophages and smooth muscle cells.	bind
30317	7	6630	6	13	NULL	NULL	NULL	GAG-induced alterations	Process		increase					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_149_s_208	9012650	14  The GAG-induced alterations are associated with an increase in LDL binding and degradation by human monocyte - derived macrophages and smooth muscle cells.	bind
30318	8	6630	6	13	NULL	NULL	NULL	GAG-induced alterations	Process		increase					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_149_s_208	9012650	14  The GAG-induced alterations are associated with an increase in LDL binding and degradation by human monocyte - derived macrophages and smooth muscle cells.	bind
56205	9	6630	6	13	NULL	NULL	NULL	macrophages	Cell		derived from					monocyte	Cell	human			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_149_s_208	9012650	14  The GAG-induced alterations are associated with an increase in LDL binding and degradation by human monocyte - derived macrophages and smooth muscle cells.	bind
21433	1	6631	5	13	NULL	NULL	NULL	 coagulation factor VII	GP		bind					tissue factor	GP				NULL	exposed on the surfaces of infiltrating cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1143_s_176	10764685	14  The generation of thrombin is thought to be initiated by coagulation factor VII/VIIa bound to tissue factor, which is exposed on the surfaces of infiltrating cells.	bind
21434	2	6631	5	13	NULL	NULL	NULL	statement 1	Process		initiates					thrombin	GP	generation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1143_s_176	10764685	14  The generation of thrombin is thought to be initiated by coagulation factor VII/VIIa bound to tissue factor, which is exposed on the surfaces of infiltrating cells.	bind
56206	3	6631	5	13	NULL	NULL	NULL	coagulation factor VIIa	GP		bind					tissue factor	GP				NULL	exposed on the surfaces of infiltrating cells.	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1143_s_176	10764685	14  The generation of thrombin is thought to be initiated by coagulation factor VII/VIIa bound to tissue factor, which is exposed on the surfaces of infiltrating cells.	bind
56207	4	6631	5	13	NULL	NULL	NULL	statement 3	Process		initiates					thrombin	GP	generation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1143_s_176	10764685	14  The generation of thrombin is thought to be initiated by coagulation factor VII/VIIa bound to tissue factor, which is exposed on the surfaces of infiltrating cells.	bind
18681	1	6631	6	13	NULL	NULL	NULL	coagulation factor VII	GP		bind					tissue factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1143_s_176	10764685	14  The generation of thrombin is thought to be initiated by coagulation factor VII/VIIa bound to tissue factor, which is exposed on the surfaces of infiltrating cells.	bind
18683	2	6631	6	13	NULL	NULL	NULL	statement 1	Process		initiates					thrombin	GP	generation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1143_s_176	10764685	14  The generation of thrombin is thought to be initiated by coagulation factor VII/VIIa bound to tissue factor, which is exposed on the surfaces of infiltrating cells.	bind
18684	3	6631	6	13	NULL	NULL	NULL	tissue factor	GP		is exposed on					surfaces of infiltrating cells	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1143_s_176	10764685	14  The generation of thrombin is thought to be initiated by coagulation factor VII/VIIa bound to tissue factor, which is exposed on the surfaces of infiltrating cells.	bind
56208	4	6631	6	13	NULL	NULL	NULL	coagulation factor VIIa	GP		bind					tissue factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1143_s_176	10764685	14  The generation of thrombin is thought to be initiated by coagulation factor VII/VIIa bound to tissue factor, which is exposed on the surfaces of infiltrating cells.	bind
56209	5	6631	6	13	NULL	NULL	NULL	statement 4	Process		initiates					thrombin	GP	generation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1143_s_176	10764685	14  The generation of thrombin is thought to be initiated by coagulation factor VII/VIIa bound to tissue factor, which is exposed on the surfaces of infiltrating cells.	bind
21438	1	6632	5	13	NULL	NULL	NULL	von Willebrand factor	GP		bind					GP Ib	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_98_8_742_s_162	9727543	14 15  Previous work suggests that the mechanism of activation involves the binding of von Willebrand factor to GP Ib, followed by an increase in cytoplasmic ionized calcium, leading to activation of the GP IIb/IIa receptor, binding of fibrinogen to GP IIb/IIa, and finally aggregation of platelets.	bind
21440	2	6632	5	13	NULL	NULL	NULL	statement 1	Process		is followed by					ionized calcium	Chemical	increase in cytoplasmic			NULL		NULL	NULL	NULL	NULL	gw60_circulation_98_8_742_s_162	9727543	14 15  Previous work suggests that the mechanism of activation involves the binding of von Willebrand factor to GP Ib, followed by an increase in cytoplasmic ionized calcium, leading to activation of the GP IIb/IIa receptor, binding of fibrinogen to GP IIb/IIa, and finally aggregation of platelets.	bind
21441	3	6632	5	13	NULL	NULL	NULL	statement 2	Process		leads to					GP IIb/IIa receptor	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_98_8_742_s_162	9727543	14 15  Previous work suggests that the mechanism of activation involves the binding of von Willebrand factor to GP Ib, followed by an increase in cytoplasmic ionized calcium, leading to activation of the GP IIb/IIa receptor, binding of fibrinogen to GP IIb/IIa, and finally aggregation of platelets.	bind
21442	4	6632	5	13	NULL	NULL	NULL	fibrinogen	GP		bind					GP IIb/IIa	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_98_8_742_s_162	9727543	14 15  Previous work suggests that the mechanism of activation involves the binding of von Willebrand factor to GP Ib, followed by an increase in cytoplasmic ionized calcium, leading to activation of the GP IIb/IIa receptor, binding of fibrinogen to GP IIb/IIa, and finally aggregation of platelets.	bind
21445	5	6632	5	13	NULL	NULL	NULL	statement 2	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_98_8_742_s_162	9727543	14 15  Previous work suggests that the mechanism of activation involves the binding of von Willebrand factor to GP Ib, followed by an increase in cytoplasmic ionized calcium, leading to activation of the GP IIb/IIa receptor, binding of fibrinogen to GP IIb/IIa, and finally aggregation of platelets.	bind
21446	6	6632	5	13	NULL	NULL	NULL	statement 2	Process		leads to		finally			platelets	Cell	aggregation of 			NULL		NULL	NULL	NULL	NULL	gw60_circulation_98_8_742_s_162	9727543	14 15  Previous work suggests that the mechanism of activation involves the binding of von Willebrand factor to GP Ib, followed by an increase in cytoplasmic ionized calcium, leading to activation of the GP IIb/IIa receptor, binding of fibrinogen to GP IIb/IIa, and finally aggregation of platelets.	bind
18686	1	6632	6	13	NULL	NULL	NULL	von Willebrand factor 	GP		bind					GP Ib	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_98_8_742_s_162	9727543	14 15  Previous work suggests that the mechanism of activation involves the binding of von Willebrand factor to GP Ib, followed by an increase in cytoplasmic ionized calcium, leading to activation of the GP IIb/IIa receptor, binding of fibrinogen to GP IIb/IIa, and finally aggregation of platelets.	bind
18687	2	6632	6	13	NULL	NULL	NULL	fibrinogen	GP		bind					GP IIb/IIa	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_98_8_742_s_162	9727543	14 15  Previous work suggests that the mechanism of activation involves the binding of von Willebrand factor to GP Ib, followed by an increase in cytoplasmic ionized calcium, leading to activation of the GP IIb/IIa receptor, binding of fibrinogen to GP IIb/IIa, and finally aggregation of platelets.	bind
18688	3	6632	6	13	NULL	NULL	NULL	cytoplasmic ionized calcium	Chemical	increase in	leads to					GP IIb/IIa receptor	GP	activation of 			NULL		NULL	NULL	NULL	NULL	gw60_circulation_98_8_742_s_162	9727543	14 15  Previous work suggests that the mechanism of activation involves the binding of von Willebrand factor to GP Ib, followed by an increase in cytoplasmic ionized calcium, leading to activation of the GP IIb/IIa receptor, binding of fibrinogen to GP IIb/IIa, and finally aggregation of platelets.	bind
18689	4	6632	6	13	NULL	NULL	NULL	statement 2	Process		leads to					aggregation of platelets	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_98_8_742_s_162	9727543	14 15  Previous work suggests that the mechanism of activation involves the binding of von Willebrand factor to GP Ib, followed by an increase in cytoplasmic ionized calcium, leading to activation of the GP IIb/IIa receptor, binding of fibrinogen to GP IIb/IIa, and finally aggregation of platelets.	bind
56210	5	6632	6	13	NULL	NULL	NULL	statement 1	Process		is followed by 					ionized calcium	Chemical	increase in cytoplasmic			NULL		NULL	NULL	NULL	NULL	gw60_circulation_98_8_742_s_162	9727543	14 15  Previous work suggests that the mechanism of activation involves the binding of von Willebrand factor to GP Ib, followed by an increase in cytoplasmic ionized calcium, leading to activation of the GP IIb/IIa receptor, binding of fibrinogen to GP IIb/IIa, and finally aggregation of platelets.	bind
56211	6	6632	6	13	NULL	NULL	NULL	statement 5	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_98_8_742_s_162	9727543	14 15  Previous work suggests that the mechanism of activation involves the binding of von Willebrand factor to GP Ib, followed by an increase in cytoplasmic ionized calcium, leading to activation of the GP IIb/IIa receptor, binding of fibrinogen to GP IIb/IIa, and finally aggregation of platelets.	bind
21447	1	6633	5	13	NULL	NULL	NULL	LDL subfractions	GP		bind					LDLRs	GP				NULL	on fibroblasts	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_6_794_s_21	8640407	14 15 16 17 18  Swinkels et al 14  found no differences in the receptor binding of LDL subfractions to LDLRs on fibroblasts and HepG2 cells, but two other studies found that both buoyant ( d=1.024 to 1.037 g/mL) and dense ( d=1.036 to 1.047 g/mL) LDL subfractions had reduced binding affinity compared with medium-density LDL subfractions ( d=1.027 to 1.041 g/mL).	bind
21448	2	6633	5	13	NULL	NULL	NULL	LDL subfractions	GP		bind					LDLRs	GP				NULL	on HepG2 cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_6_794_s_21	8640407	14 15 16 17 18  Swinkels et al 14  found no differences in the receptor binding of LDL subfractions to LDLRs on fibroblasts and HepG2 cells, but two other studies found that both buoyant ( d=1.024 to 1.037 g/mL) and dense ( d=1.036 to 1.047 g/mL) LDL subfractions had reduced binding affinity compared with medium-density LDL subfractions ( d=1.027 to 1.041 g/mL).	bind
24765	3	6633	5	13	NULL	NULL	NULL	statement 1	Process	binding of	is not different from					statement 2	Process	binding of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_6_794_s_21	8640407	14 15 16 17 18  Swinkels et al 14  found no differences in the receptor binding of LDL subfractions to LDLRs on fibroblasts and HepG2 cells, but two other studies found that both buoyant ( d=1.024 to 1.037 g/mL) and dense ( d=1.036 to 1.047 g/mL) LDL subfractions had reduced binding affinity compared with medium-density LDL subfractions ( d=1.027 to 1.041 g/mL).	bind
24766	4	6633	5	13	NULL	NULL	NULL	LDL subfractions	GP	buoyant	bind					LDLRs	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_6_794_s_21	8640407	14 15 16 17 18  Swinkels et al 14  found no differences in the receptor binding of LDL subfractions to LDLRs on fibroblasts and HepG2 cells, but two other studies found that both buoyant ( d=1.024 to 1.037 g/mL) and dense ( d=1.036 to 1.047 g/mL) LDL subfractions had reduced binding affinity compared with medium-density LDL subfractions ( d=1.027 to 1.041 g/mL).	bind
24769	5	6633	5	13	NULL	NULL	NULL	LDL subfractions	GP	dense	bind					LDLRs	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_6_794_s_21	8640407	14 15 16 17 18  Swinkels et al 14  found no differences in the receptor binding of LDL subfractions to LDLRs on fibroblasts and HepG2 cells, but two other studies found that both buoyant ( d=1.024 to 1.037 g/mL) and dense ( d=1.036 to 1.047 g/mL) LDL subfractions had reduced binding affinity compared with medium-density LDL subfractions ( d=1.027 to 1.041 g/mL).	bind
24772	6	6633	5	13	NULL	NULL	NULL	LDL subfractions	GP	medium-density	bind					LDLRs	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_6_794_s_21	8640407	14 15 16 17 18  Swinkels et al 14  found no differences in the receptor binding of LDL subfractions to LDLRs on fibroblasts and HepG2 cells, but two other studies found that both buoyant ( d=1.024 to 1.037 g/mL) and dense ( d=1.036 to 1.047 g/mL) LDL subfractions had reduced binding affinity compared with medium-density LDL subfractions ( d=1.027 to 1.041 g/mL).	bind
24773	7	6633	5	13	NULL	NULL	NULL	statement 4	Process		reduced affinity than					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_6_794_s_21	8640407	14 15 16 17 18  Swinkels et al 14  found no differences in the receptor binding of LDL subfractions to LDLRs on fibroblasts and HepG2 cells, but two other studies found that both buoyant ( d=1.024 to 1.037 g/mL) and dense ( d=1.036 to 1.047 g/mL) LDL subfractions had reduced binding affinity compared with medium-density LDL subfractions ( d=1.027 to 1.041 g/mL).	bind
24774	8	6633	5	13	NULL	NULL	NULL	statement 5	Process		reduced affinity than					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_6_794_s_21	8640407	14 15 16 17 18  Swinkels et al 14  found no differences in the receptor binding of LDL subfractions to LDLRs on fibroblasts and HepG2 cells, but two other studies found that both buoyant ( d=1.024 to 1.037 g/mL) and dense ( d=1.036 to 1.047 g/mL) LDL subfractions had reduced binding affinity compared with medium-density LDL subfractions ( d=1.027 to 1.041 g/mL).	bind
18708	1	6633	6	13	NULL	NULL	NULL	LDL subfraction	GP		bind					LDLR	GP				NULL	fibroblasts	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_6_794_s_21	8640407	14 15 16 17 18  Swinkels et al 14  found no differences in the receptor binding of LDL subfractions to LDLRs on fibroblasts and HepG2 cells, but two other studies found that both buoyant ( d=1.024 to 1.037 g/mL) and dense ( d=1.036 to 1.047 g/mL) LDL subfractions had reduced binding affinity compared with medium-density LDL subfractions ( d=1.027 to 1.041 g/mL).	bind
18709	2	6633	6	13	NULL	NULL	NULL	LDL subfraction	GP		bind					LDLR	GP				NULL	HepG2 cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_6_794_s_21	8640407	14 15 16 17 18  Swinkels et al 14  found no differences in the receptor binding of LDL subfractions to LDLRs on fibroblasts and HepG2 cells, but two other studies found that both buoyant ( d=1.024 to 1.037 g/mL) and dense ( d=1.036 to 1.047 g/mL) LDL subfractions had reduced binding affinity compared with medium-density LDL subfractions ( d=1.027 to 1.041 g/mL).	bind
18710	3	6633	6	13	NULL	NULL	NULL	LDL subfraction	GP	buoyant	bind					LDLR	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_6_794_s_21	8640407	14 15 16 17 18  Swinkels et al 14  found no differences in the receptor binding of LDL subfractions to LDLRs on fibroblasts and HepG2 cells, but two other studies found that both buoyant ( d=1.024 to 1.037 g/mL) and dense ( d=1.036 to 1.047 g/mL) LDL subfractions had reduced binding affinity compared with medium-density LDL subfractions ( d=1.027 to 1.041 g/mL).	bind
18711	4	6633	6	13	NULL	NULL	NULL	LDL subfraction	GP	dense	bind					LDLR	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_6_794_s_21	8640407	14 15 16 17 18  Swinkels et al 14  found no differences in the receptor binding of LDL subfractions to LDLRs on fibroblasts and HepG2 cells, but two other studies found that both buoyant ( d=1.024 to 1.037 g/mL) and dense ( d=1.036 to 1.047 g/mL) LDL subfractions had reduced binding affinity compared with medium-density LDL subfractions ( d=1.027 to 1.041 g/mL).	bind
30274	5	6633	6	13	NULL	NULL	NULL	LDL subfraction	GP	medium	bind					LDLR	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_6_794_s_21	8640407	14 15 16 17 18  Swinkels et al 14  found no differences in the receptor binding of LDL subfractions to LDLRs on fibroblasts and HepG2 cells, but two other studies found that both buoyant ( d=1.024 to 1.037 g/mL) and dense ( d=1.036 to 1.047 g/mL) LDL subfractions had reduced binding affinity compared with medium-density LDL subfractions ( d=1.027 to 1.041 g/mL).	bind
30275	6	6633	6	13	NULL	NULL	NULL	statement 3	Process	affinity of	is reduced in comparision with					statement 5	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_6_794_s_21	8640407	14 15 16 17 18  Swinkels et al 14  found no differences in the receptor binding of LDL subfractions to LDLRs on fibroblasts and HepG2 cells, but two other studies found that both buoyant ( d=1.024 to 1.037 g/mL) and dense ( d=1.036 to 1.047 g/mL) LDL subfractions had reduced binding affinity compared with medium-density LDL subfractions ( d=1.027 to 1.041 g/mL).	bind
30276	7	6633	6	13	NULL	NULL	NULL	statement 4	Process	affinity of	is reduced in comparision with					statement 5	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_6_794_s_21	8640407	14 15 16 17 18  Swinkels et al 14  found no differences in the receptor binding of LDL subfractions to LDLRs on fibroblasts and HepG2 cells, but two other studies found that both buoyant ( d=1.024 to 1.037 g/mL) and dense ( d=1.036 to 1.047 g/mL) LDL subfractions had reduced binding affinity compared with medium-density LDL subfractions ( d=1.027 to 1.041 g/mL).	bind
56212	8	6633	6	13	NULL	NULL	NULL	statement 1	Process	binding of	is not different from					statement 2	Process	binding of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_6_794_s_21	8640407	14 15 16 17 18  Swinkels et al 14  found no differences in the receptor binding of LDL subfractions to LDLRs on fibroblasts and HepG2 cells, but two other studies found that both buoyant ( d=1.024 to 1.037 g/mL) and dense ( d=1.036 to 1.047 g/mL) LDL subfractions had reduced binding affinity compared with medium-density LDL subfractions ( d=1.027 to 1.041 g/mL).	bind
21449	1	6634	5	13	NULL	NULL	NULL	CA-4	GP		bind					tubulin	GP		colchicine binding site		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_1097_s_151	11891206	14 Although the mechanism of action giving rise to this effect remains to be elucidated, it has been proposed that CA-4, which binds to the colchicine binding site of tubulin, elicits a shape change in the endothelial cells of tumor vessels that compromises the integrity of the lumenal monolayer.	bind
21450	2	6634	5	13	NULL	NULL	NULL	CA-4	GP		elicits					endothelial cells	Cell	shape change			NULL	of tumor vessels	NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_1097_s_151	11891206	14 Although the mechanism of action giving rise to this effect remains to be elucidated, it has been proposed that CA-4, which binds to the colchicine binding site of tubulin, elicits a shape change in the endothelial cells of tumor vessels that compromises the integrity of the lumenal monolayer.	bind
21451	3	6634	5	13	NULL	NULL	NULL	statement 2	Process		compromises					lumenal monolayer	OrganismPart	integrity of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_1097_s_151	11891206	14 Although the mechanism of action giving rise to this effect remains to be elucidated, it has been proposed that CA-4, which binds to the colchicine binding site of tubulin, elicits a shape change in the endothelial cells of tumor vessels that compromises the integrity of the lumenal monolayer.	bind
18712	1	6634	6	13	NULL	NULL	NULL	CA-4	GP		bind					tubulin	GP		colchicine binding site		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_1097_s_151	11891206	14 Although the mechanism of action giving rise to this effect remains to be elucidated, it has been proposed that CA-4, which binds to the colchicine binding site of tubulin, elicits a shape change in the endothelial cells of tumor vessels that compromises the integrity of the lumenal monolayer.	bind
18713	2	6634	6	13	NULL	NULL	NULL	CA-4	GP		elicits					endothelial  cells	Cell	shape change of			NULL	tumour vessels	NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_1097_s_151	11891206	14 Although the mechanism of action giving rise to this effect remains to be elucidated, it has been proposed that CA-4, which binds to the colchicine binding site of tubulin, elicits a shape change in the endothelial cells of tumor vessels that compromises the integrity of the lumenal monolayer.	bind
18714	3	6634	6	13	NULL	NULL	NULL	statement 2	Process		compromises					lumenal monolayer	OrganismPart	integrity of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_1097_s_151	11891206	14 Although the mechanism of action giving rise to this effect remains to be elucidated, it has been proposed that CA-4, which binds to the colchicine binding site of tubulin, elicits a shape change in the endothelial cells of tumor vessels that compromises the integrity of the lumenal monolayer.	bind
21452	1	6635	5	13	NULL	NULL	NULL	PS1	GP		associates with					E-cadherin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_5_2381_s_62	11226248	14 and  22), our data show that PS1 associates with E-cadherin even when catenins are not bound to E-cadherin.	bind
21453	2	6635	5	13	NULL	NULL	NULL	catenins	GP		bind					E-cadherin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_5_2381_s_62	11226248	14 and  22), our data show that PS1 associates with E-cadherin even when catenins are not bound to E-cadherin.	bind
21454	3	6635	5	13	NULL	NULL	NULL	statement 1	Process		in the absence of					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_5_2381_s_62	11226248	14 and  22), our data show that PS1 associates with E-cadherin even when catenins are not bound to E-cadherin.	bind
18715	1	6635	6	13	NULL	NULL	NULL	PS1	GP		associates with					E-cadherin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_5_2381_s_62	11226248	14 and  22), our data show that PS1 associates with E-cadherin even when catenins are not bound to E-cadherin.	bind
18716	2	6635	6	13	NULL	NULL	NULL	catenin	GP		does not bind					E-cadherin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_5_2381_s_62	11226248	14 and  22), our data show that PS1 associates with E-cadherin even when catenins are not bound to E-cadherin.	bind
18717	3	6635	6	13	NULL	NULL	NULL	statement 1	Process		occurs irrespective of					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_5_2381_s_62	11226248	14 and  22), our data show that PS1 associates with E-cadherin even when catenins are not bound to E-cadherin.	bind
21455	1	6636	5	13	NULL	NULL	NULL	laminin 5	GP		dimerizes with					laminin 6	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_2_459_s_18	11839566	14 Instead, laminin 5 forms a dimer with laminin 6 or 7 18  and binds to collagen VII. 19, 20  In addition, laminin 5 is synthesized as a 460-kd precursor that is extracellularly converted into tissular forms of 440- and 400-kd by enzymatic processing.	bind
21456	2	6636	5	13	NULL	NULL	NULL	laminin 5	GP		dimerizes with					laminin 7	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_2_459_s_18	11839566	14 Instead, laminin 5 forms a dimer with laminin 6 or 7 18  and binds to collagen VII. 19, 20  In addition, laminin 5 is synthesized as a 460-kd precursor that is extracellularly converted into tissular forms of 440- and 400-kd by enzymatic processing.	bind
21457	3	6636	5	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_2_459_s_18	11839566	14 Instead, laminin 5 forms a dimer with laminin 6 or 7 18  and binds to collagen VII. 19, 20  In addition, laminin 5 is synthesized as a 460-kd precursor that is extracellularly converted into tissular forms of 440- and 400-kd by enzymatic processing.	bind
21458	4	6636	5	13	NULL	NULL	NULL	laminin 5	GP		bind					collagen VII	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_2_459_s_18	11839566	14 Instead, laminin 5 forms a dimer with laminin 6 or 7 18  and binds to collagen VII. 19, 20  In addition, laminin 5 is synthesized as a 460-kd precursor that is extracellularly converted into tissular forms of 440- and 400-kd by enzymatic processing.	bind
21461	5	6636	5	13	NULL	NULL	NULL	laminin 5	GP	precursor	is converted into		extracellularly			tissular forms					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_2_459_s_18	11839566	14 Instead, laminin 5 forms a dimer with laminin 6 or 7 18  and binds to collagen VII. 19, 20  In addition, laminin 5 is synthesized as a 460-kd precursor that is extracellularly converted into tissular forms of 440- and 400-kd by enzymatic processing.	bind
21462	6	6636	5	13	NULL	NULL	NULL	enzymatic processing	Process		is required for					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_2_459_s_18	11839566	14 Instead, laminin 5 forms a dimer with laminin 6 or 7 18  and binds to collagen VII. 19, 20  In addition, laminin 5 is synthesized as a 460-kd precursor that is extracellularly converted into tissular forms of 440- and 400-kd by enzymatic processing.	bind
18718	1	6636	6	13	NULL	NULL	NULL	laminin 5	GP		forms a dimer with					laminin 6	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_2_459_s_18	11839566	14 Instead, laminin 5 forms a dimer with laminin 6 or 7 18  and binds to collagen VII. 19, 20  In addition, laminin 5 is synthesized as a 460-kd precursor that is extracellularly converted into tissular forms of 440- and 400-kd by enzymatic processing.	bind
18719	2	6636	6	13	NULL	NULL	NULL	laminin 5	GP		forms a dimer with					laminin 7	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_2_459_s_18	11839566	14 Instead, laminin 5 forms a dimer with laminin 6 or 7 18  and binds to collagen VII. 19, 20  In addition, laminin 5 is synthesized as a 460-kd precursor that is extracellularly converted into tissular forms of 440- and 400-kd by enzymatic processing.	bind
18720	3	6636	6	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_2_459_s_18	11839566	14 Instead, laminin 5 forms a dimer with laminin 6 or 7 18  and binds to collagen VII. 19, 20  In addition, laminin 5 is synthesized as a 460-kd precursor that is extracellularly converted into tissular forms of 440- and 400-kd by enzymatic processing.	bind
18721	4	6636	6	13	NULL	NULL	NULL	laminin 5	GP		bind					collagen VII	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_2_459_s_18	11839566	14 Instead, laminin 5 forms a dimer with laminin 6 or 7 18  and binds to collagen VII. 19, 20  In addition, laminin 5 is synthesized as a 460-kd precursor that is extracellularly converted into tissular forms of 440- and 400-kd by enzymatic processing.	bind
56213	5	6636	6	13	NULL	NULL	NULL	laminin 5	GP	precursor	coverted to		extracellularly			tissular forms					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_2_459_s_18	11839566	14 Instead, laminin 5 forms a dimer with laminin 6 or 7 18  and binds to collagen VII. 19, 20  In addition, laminin 5 is synthesized as a 460-kd precursor that is extracellularly converted into tissular forms of 440- and 400-kd by enzymatic processing.	bind
56214	6	6636	6	13	NULL	NULL	NULL	enzymatic processing	Process		is required for					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_2_459_s_18	11839566	14 Instead, laminin 5 forms a dimer with laminin 6 or 7 18  and binds to collagen VII. 19, 20  In addition, laminin 5 is synthesized as a 460-kd precursor that is extracellularly converted into tissular forms of 440- and 400-kd by enzymatic processing.	bind
21463	1	6637	5	13	NULL	NULL	NULL	Sp1	GP		bind									Sp1 motif	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_12_1202_s_225	14593001	14 It has been proposed that Sp3 competes with Sp1 binding to the Sp1 motif and thus serves as negative regulator of Sp1 sites.	bind
21464	2	6637	5	13	NULL	NULL	NULL	Sp3	GP		bind									Sp1 motif	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_12_1202_s_225	14593001	14 It has been proposed that Sp3 competes with Sp1 binding to the Sp1 motif and thus serves as negative regulator of Sp1 sites.	bind
21465	3	6637	5	13	NULL	NULL	NULL	statement 2	Process		competes with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_12_1202_s_225	14593001	14 It has been proposed that Sp3 competes with Sp1 binding to the Sp1 motif and thus serves as negative regulator of Sp1 sites.	bind
21466	4	6637	5	13	NULL	NULL	NULL	Sp3	GP		regulates		negatively							Sp1 sites	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_12_1202_s_225	14593001	14 It has been proposed that Sp3 competes with Sp1 binding to the Sp1 motif and thus serves as negative regulator of Sp1 sites.	bind
21467	5	6637	5	13	NULL	NULL	NULL	statement 3	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_12_1202_s_225	14593001	14 It has been proposed that Sp3 competes with Sp1 binding to the Sp1 motif and thus serves as negative regulator of Sp1 sites.	bind
18722	1	6637	6	13	NULL	NULL	NULL	Sp1	GP		bind									Sp1 motif	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_12_1202_s_225	14593001	14 It has been proposed that Sp3 competes with Sp1 binding to the Sp1 motif and thus serves as negative regulator of Sp1 sites.	bind
18723	2	6637	6	13	NULL	NULL	NULL	Sp3	GP		bind									Sp1 motif	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_12_1202_s_225	14593001	14 It has been proposed that Sp3 competes with Sp1 binding to the Sp1 motif and thus serves as negative regulator of Sp1 sites.	bind
18724	3	6637	6	13	NULL	NULL	NULL	statement 1	Process		competes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_12_1202_s_225	14593001	14 It has been proposed that Sp3 competes with Sp1 binding to the Sp1 motif and thus serves as negative regulator of Sp1 sites.	bind
18725	4	6637	6	13	NULL	NULL	NULL	Sp3	GP		regulates		negatively 							Sp1 sites	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_12_1202_s_225	14593001	14 It has been proposed that Sp3 competes with Sp1 binding to the Sp1 motif and thus serves as negative regulator of Sp1 sites.	bind
30273	5	6637	6	13	NULL	NULL	NULL	statement 3	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_12_1202_s_225	14593001	14 It has been proposed that Sp3 competes with Sp1 binding to the Sp1 motif and thus serves as negative regulator of Sp1 sites.	bind
21468	1	6638	5	13	NULL	NULL	NULL	CYP2C9	GP		increase					COX-2	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_321_s_170	15569819	14 Moreover, the CYP2C9-induced increase in COX-2 expression reported here also depends on an increase in the DNA binding of CREB to the COX-2 promoter.	bind
21469	2	6638	5	13	NULL	NULL	NULL	CREB	GP		bind					COX-2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_321_s_170	15569819	14 Moreover, the CYP2C9-induced increase in COX-2 expression reported here also depends on an increase in the DNA binding of CREB to the COX-2 promoter.	bind
21470	3	6638	5	13	NULL	NULL	NULL	statement 1	Process		depends upon					statement 2	Process	increase in			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_321_s_170	15569819	14 Moreover, the CYP2C9-induced increase in COX-2 expression reported here also depends on an increase in the DNA binding of CREB to the COX-2 promoter.	bind
18726	1	6638	6	13	NULL	NULL	NULL	CYP2C9	GP		increase					COX-2	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_321_s_170	15569819	14 Moreover, the CYP2C9-induced increase in COX-2 expression reported here also depends on an increase in the DNA binding of CREB to the COX-2 promoter.	bind
18727	2	6638	6	13	NULL	NULL	NULL	CREB	GP		bind					COX-2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_321_s_170	15569819	14 Moreover, the CYP2C9-induced increase in COX-2 expression reported here also depends on an increase in the DNA binding of CREB to the COX-2 promoter.	bind
30272	3	6638	6	13	NULL	NULL	NULL	statement 1	Process		depends on					statement 2	Process	increase in			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_321_s_170	15569819	14 Moreover, the CYP2C9-induced increase in COX-2 expression reported here also depends on an increase in the DNA binding of CREB to the COX-2 promoter.	bind
21471	1	6639	5	13	NULL	NULL	NULL	MR	GP		bind									glucocorticoid response elements	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_circulationres_96_6_643_s_35	15718497	14 MR binds in vitro to glucocorticoid and mineralocorticoid response elements in a ligand-dependent manner.	bind
21472	2	6639	5	13	NULL	NULL	NULL	statement 1	Process		is dependent on					ligand	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_6_643_s_35	15718497	14 MR binds in vitro to glucocorticoid and mineralocorticoid response elements in a ligand-dependent manner.	bind
21473	3	6639	5	13	NULL	NULL	NULL	MR	GP		bind									mineralocorticoid response elements	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_circulationres_96_6_643_s_35	15718497	14 MR binds in vitro to glucocorticoid and mineralocorticoid response elements in a ligand-dependent manner.	bind
21474	4	6639	5	13	NULL	NULL	NULL	statement 3	Process		is dependent on					ligand	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_6_643_s_35	15718497	14 MR binds in vitro to glucocorticoid and mineralocorticoid response elements in a ligand-dependent manner.	bind
18728	1	6639	6	13	NULL	NULL	NULL	MR	GP		bind									glucocorticoid responsive element	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_circulationres_96_6_643_s_35	15718497	14 MR binds in vitro to glucocorticoid and mineralocorticoid response elements in a ligand-dependent manner.	bind
18729	2	6639	6	13	NULL	NULL	NULL	MR	GP		bind									mineralocorticoid response element	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_circulationres_96_6_643_s_35	15718497	14 MR binds in vitro to glucocorticoid and mineralocorticoid response elements in a ligand-dependent manner.	bind
18730	3	6639	6	13	NULL	NULL	NULL	statement 1	Process		is dependent on					ligand	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_6_643_s_35	15718497	14 MR binds in vitro to glucocorticoid and mineralocorticoid response elements in a ligand-dependent manner.	bind
18731	4	6639	6	13	NULL	NULL	NULL	statement 2	Process		is dependent on					ligand	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_6_643_s_35	15718497	14 MR binds in vitro to glucocorticoid and mineralocorticoid response elements in a ligand-dependent manner.	bind
24775	1	6640	5	13	NULL	NULL	NULL	Flt-sel	GP		elicits		potently			PAE	Cell	migration of			NULL	in PAE cells transfected with an Flt-1 mutant receptor	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_12_1934_s_191	11742867	14 Recently Gille et al 15 showed that Flt-sel could potently elicit PAE migration by using PAE cells transfected with an Flt-1 mutant receptor in which 3 amino acids of the juxtamembrane region were exchanged with KDR. 30 Finally, the lack of response to PLGF, a naturally occurring VEGF family member that selectively binds Flt-1, further substantiates the differential roles of KDR versus Flt-1 in endothelial tube formation.	bind
24776	2	6640	5	13	NULL	NULL	NULL	Flt-1 receptor	GP	mutant	is exchanged with			3 amino acids of the juxtamembrane region		KDR	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_12_1934_s_191	11742867	14 Recently Gille et al 15 showed that Flt-sel could potently elicit PAE migration by using PAE cells transfected with an Flt-1 mutant receptor in which 3 amino acids of the juxtamembrane region were exchanged with KDR. 30 Finally, the lack of response to PLGF, a naturally occurring VEGF family member that selectively binds Flt-1, further substantiates the differential roles of KDR versus Flt-1 in endothelial tube formation.	bind
24777	3	6640	5	13	NULL	NULL	NULL	PLGF	GP		is a member of					VEGF family	GP	naturally occurring			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_12_1934_s_191	11742867	14 Recently Gille et al 15 showed that Flt-sel could potently elicit PAE migration by using PAE cells transfected with an Flt-1 mutant receptor in which 3 amino acids of the juxtamembrane region were exchanged with KDR. 30 Finally, the lack of response to PLGF, a naturally occurring VEGF family member that selectively binds Flt-1, further substantiates the differential roles of KDR versus Flt-1 in endothelial tube formation.	bind
24778	4	6640	5	13	NULL	NULL	NULL	PLGF	GP		bind		selectively			Flt-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_12_1934_s_191	11742867	14 Recently Gille et al 15 showed that Flt-sel could potently elicit PAE migration by using PAE cells transfected with an Flt-1 mutant receptor in which 3 amino acids of the juxtamembrane region were exchanged with KDR. 30 Finally, the lack of response to PLGF, a naturally occurring VEGF family member that selectively binds Flt-1, further substantiates the differential roles of KDR versus Flt-1 in endothelial tube formation.	bind
24781	5	6640	5	13	NULL	NULL	NULL	KDR	GP		plays a role in		differential			endothelial tube	OrganismPart	formation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_12_1934_s_191	11742867	14 Recently Gille et al 15 showed that Flt-sel could potently elicit PAE migration by using PAE cells transfected with an Flt-1 mutant receptor in which 3 amino acids of the juxtamembrane region were exchanged with KDR. 30 Finally, the lack of response to PLGF, a naturally occurring VEGF family member that selectively binds Flt-1, further substantiates the differential roles of KDR versus Flt-1 in endothelial tube formation.	bind
24782	6	6640	5	13	NULL	NULL	NULL	Flt-1	GP		plays a role in		differential			endothelial tube	OrganismPart	formation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_12_1934_s_191	11742867	14 Recently Gille et al 15 showed that Flt-sel could potently elicit PAE migration by using PAE cells transfected with an Flt-1 mutant receptor in which 3 amino acids of the juxtamembrane region were exchanged with KDR. 30 Finally, the lack of response to PLGF, a naturally occurring VEGF family member that selectively binds Flt-1, further substantiates the differential roles of KDR versus Flt-1 in endothelial tube formation.	bind
24784	7	6640	5	13	NULL	NULL	NULL	PLGF	GP	lack of response to	substantiates					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_12_1934_s_191	11742867	14 Recently Gille et al 15 showed that Flt-sel could potently elicit PAE migration by using PAE cells transfected with an Flt-1 mutant receptor in which 3 amino acids of the juxtamembrane region were exchanged with KDR. 30 Finally, the lack of response to PLGF, a naturally occurring VEGF family member that selectively binds Flt-1, further substantiates the differential roles of KDR versus Flt-1 in endothelial tube formation.	bind
24786	8	6640	5	13	NULL	NULL	NULL	PLGF	GP	lack of response to	substantiates					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_12_1934_s_191	11742867	14 Recently Gille et al 15 showed that Flt-sel could potently elicit PAE migration by using PAE cells transfected with an Flt-1 mutant receptor in which 3 amino acids of the juxtamembrane region were exchanged with KDR. 30 Finally, the lack of response to PLGF, a naturally occurring VEGF family member that selectively binds Flt-1, further substantiates the differential roles of KDR versus Flt-1 in endothelial tube formation.	bind
18732	1	6640	6	13	NULL	NULL	NULL	Flt-sel	GP		elicit 		potentially			PAE	Cell	migration of			NULL	PAE cells transfected with an Flt-1 mutant receptor	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_12_1934_s_191	11742867	14 Recently Gille et al 15 showed that Flt-sel could potently elicit PAE migration by using PAE cells transfected with an Flt-1 mutant receptor in which 3 amino acids of the juxtamembrane region were exchanged with KDR. 30 Finally, the lack of response to PLGF, a naturally occurring VEGF family member that selectively binds Flt-1, further substantiates the differential roles of KDR versus Flt-1 in endothelial tube formation.	bind
18733	2	6640	6	13	NULL	NULL	NULL	PLGF	GP		bind		selectively			Flt-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_12_1934_s_191	11742867	14 Recently Gille et al 15 showed that Flt-sel could potently elicit PAE migration by using PAE cells transfected with an Flt-1 mutant receptor in which 3 amino acids of the juxtamembrane region were exchanged with KDR. 30 Finally, the lack of response to PLGF, a naturally occurring VEGF family member that selectively binds Flt-1, further substantiates the differential roles of KDR versus Flt-1 in endothelial tube formation.	bind
18734	3	6640	6	13	NULL	NULL	NULL	Flt-1	GP		plays a role in		differential			endothelial tube 	OrganismPart	formation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_12_1934_s_191	11742867	14 Recently Gille et al 15 showed that Flt-sel could potently elicit PAE migration by using PAE cells transfected with an Flt-1 mutant receptor in which 3 amino acids of the juxtamembrane region were exchanged with KDR. 30 Finally, the lack of response to PLGF, a naturally occurring VEGF family member that selectively binds Flt-1, further substantiates the differential roles of KDR versus Flt-1 in endothelial tube formation.	bind
56215	4	6640	6	13	NULL	NULL	NULL	Flt-1 receptor	GP	mutant	exchanged with			3 amino acids of the juxtamembrane region		KDR	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_12_1934_s_191	11742867	14 Recently Gille et al 15 showed that Flt-sel could potently elicit PAE migration by using PAE cells transfected with an Flt-1 mutant receptor in which 3 amino acids of the juxtamembrane region were exchanged with KDR. 30 Finally, the lack of response to PLGF, a naturally occurring VEGF family member that selectively binds Flt-1, further substantiates the differential roles of KDR versus Flt-1 in endothelial tube formation.	bind
56216	5	6640	6	13	NULL	NULL	NULL	KDR	GP		play role in		differential			endothelial tube	OrganismPart	formation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_12_1934_s_191	11742867	14 Recently Gille et al 15 showed that Flt-sel could potently elicit PAE migration by using PAE cells transfected with an Flt-1 mutant receptor in which 3 amino acids of the juxtamembrane region were exchanged with KDR. 30 Finally, the lack of response to PLGF, a naturally occurring VEGF family member that selectively binds Flt-1, further substantiates the differential roles of KDR versus Flt-1 in endothelial tube formation.	bind
56218	6	6640	6	13	NULL	NULL	NULL	PLGF	GP		is a member of					VEGF family	GP	naturally occurring			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_12_1934_s_191	11742867	14 Recently Gille et al 15 showed that Flt-sel could potently elicit PAE migration by using PAE cells transfected with an Flt-1 mutant receptor in which 3 amino acids of the juxtamembrane region were exchanged with KDR. 30 Finally, the lack of response to PLGF, a naturally occurring VEGF family member that selectively binds Flt-1, further substantiates the differential roles of KDR versus Flt-1 in endothelial tube formation.	bind
56219	7	6640	6	13	NULL	NULL	NULL	PLGF	GP	lack of response to	substantiates					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_12_1934_s_191	11742867	14 Recently Gille et al 15 showed that Flt-sel could potently elicit PAE migration by using PAE cells transfected with an Flt-1 mutant receptor in which 3 amino acids of the juxtamembrane region were exchanged with KDR. 30 Finally, the lack of response to PLGF, a naturally occurring VEGF family member that selectively binds Flt-1, further substantiates the differential roles of KDR versus Flt-1 in endothelial tube formation.	bind
56220	8	6640	6	13	NULL	NULL	NULL	PLGF	GP	lack of response to	substantiates					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_12_1934_s_191	11742867	14 Recently Gille et al 15 showed that Flt-sel could potently elicit PAE migration by using PAE cells transfected with an Flt-1 mutant receptor in which 3 amino acids of the juxtamembrane region were exchanged with KDR. 30 Finally, the lack of response to PLGF, a naturally occurring VEGF family member that selectively binds Flt-1, further substantiates the differential roles of KDR versus Flt-1 in endothelial tube formation.	bind
21475	1	6641	5	13	NULL	NULL	NULL	DDAH2	GP		bind		directly			PKA	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1419_s_29	16794231	14 Surprisingly, the mechanism is not via increased NO production, as had been previously assumed, but by the direct binding of DDAH2 to protein kinase A (PKA) and subsequent phosphorylation of the transcription factor Sp1.	bind
21476	2	6641	5	13	NULL	NULL	NULL	PKA	GP		is					protein kinase A	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1419_s_29	16794231	14 Surprisingly, the mechanism is not via increased NO production, as had been previously assumed, but by the direct binding of DDAH2 to protein kinase A (PKA) and subsequent phosphorylation of the transcription factor Sp1.	bind
21477	3	6641	5	13	NULL	NULL	NULL	statement 1	Process		phosphorylate		subsequently			Sp1	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1419_s_29	16794231	14 Surprisingly, the mechanism is not via increased NO production, as had been previously assumed, but by the direct binding of DDAH2 to protein kinase A (PKA) and subsequent phosphorylation of the transcription factor Sp1.	bind
30339	4	6641	5	13	NULL	NULL	NULL	Sp1	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1419_s_29	16794231	14 Surprisingly, the mechanism is not via increased NO production, as had been previously assumed, but by the direct binding of DDAH2 to protein kinase A (PKA) and subsequent phosphorylation of the transcription factor Sp1.	bind
18735	1	6641	6	13	NULL	NULL	NULL	DDAH2	GP		bind		directly			PKA	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1419_s_29	16794231	14 Surprisingly, the mechanism is not via increased NO production, as had been previously assumed, but by the direct binding of DDAH2 to protein kinase A (PKA) and subsequent phosphorylation of the transcription factor Sp1.	bind
18736	2	6641	6	13	NULL	NULL	NULL	PKA	GP		is					protein kinase A	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1419_s_29	16794231	14 Surprisingly, the mechanism is not via increased NO production, as had been previously assumed, but by the direct binding of DDAH2 to protein kinase A (PKA) and subsequent phosphorylation of the transcription factor Sp1.	bind
18737	3	6641	6	13	NULL	NULL	NULL	statement 1	Process		phosphorylate					Sp1	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1419_s_29	16794231	14 Surprisingly, the mechanism is not via increased NO production, as had been previously assumed, but by the direct binding of DDAH2 to protein kinase A (PKA) and subsequent phosphorylation of the transcription factor Sp1.	bind
30458	4	6641	6	13	NULL	NULL	NULL	Sp1	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1419_s_29	16794231	14 Surprisingly, the mechanism is not via increased NO production, as had been previously assumed, but by the direct binding of DDAH2 to protein kinase A (PKA) and subsequent phosphorylation of the transcription factor Sp1.	bind
21478	1	6642	5	13	NULL	NULL	NULL	syndecan-4	GP		bind		specifically	extracellular domain		foreskin fibroblasts	Cell	human			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_5_488_s_45	15774861	14 The extracellular domain of syndecan-4 binds specifically to human foreskin fibroblasts (IC50=10 - 8 M) and mouse aortic endothelial cells, as well as other cell types, whereas same-species syndecan family members did not efficiently compete with these interactions.	bind
21479	2	6642	5	13	NULL	NULL	NULL	syndecan-4	GP		bind		specifically	extracellular domain		aortic endothelial cells	Cell	mouse			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_5_488_s_45	15774861	14 The extracellular domain of syndecan-4 binds specifically to human foreskin fibroblasts (IC50=10 - 8 M) and mouse aortic endothelial cells, as well as other cell types, whereas same-species syndecan family members did not efficiently compete with these interactions.	bind
21480	3	6642	5	13	NULL	NULL	NULL	same-species syndecan family members	GP		does not compete with		efficiently			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_5_488_s_45	15774861	14 The extracellular domain of syndecan-4 binds specifically to human foreskin fibroblasts (IC50=10 - 8 M) and mouse aortic endothelial cells, as well as other cell types, whereas same-species syndecan family members did not efficiently compete with these interactions.	bind
21481	4	6642	5	13	NULL	NULL	NULL	same-species syndecan family members	GP		does not compete with		efficiently			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_5_488_s_45	15774861	14 The extracellular domain of syndecan-4 binds specifically to human foreskin fibroblasts (IC50=10 - 8 M) and mouse aortic endothelial cells, as well as other cell types, whereas same-species syndecan family members did not efficiently compete with these interactions.	bind
18738	1	6642	6	13	NULL	NULL	NULL	syndecan-4	GP		bind		specifically	extracellular domain		foreskin fibroblasts	Cell	human			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_5_488_s_45	15774861	14 The extracellular domain of syndecan-4 binds specifically to human foreskin fibroblasts (IC50=10 - 8 M) and mouse aortic endothelial cells, as well as other cell types, whereas same-species syndecan family members did not efficiently compete with these interactions.	bind
18739	2	6642	6	13	NULL	NULL	NULL	syndecan-4	GP		bind		specifically	extracellular domain		aortic endothelial cells	Cell	mouse			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_5_488_s_45	15774861	14 The extracellular domain of syndecan-4 binds specifically to human foreskin fibroblasts (IC50=10 - 8 M) and mouse aortic endothelial cells, as well as other cell types, whereas same-species syndecan family members did not efficiently compete with these interactions.	bind
30459	3	6642	6	13	NULL	NULL	NULL	same-species syndecan family members	GP		does not compete with		efficiently			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_5_488_s_45	15774861	14 The extracellular domain of syndecan-4 binds specifically to human foreskin fibroblasts (IC50=10 - 8 M) and mouse aortic endothelial cells, as well as other cell types, whereas same-species syndecan family members did not efficiently compete with these interactions.	bind
30460	4	6642	6	13	NULL	NULL	NULL	same-species syndecan family members	GP		does not compete with		efficiently			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_5_488_s_45	15774861	14 The extracellular domain of syndecan-4 binds specifically to human foreskin fibroblasts (IC50=10 - 8 M) and mouse aortic endothelial cells, as well as other cell types, whereas same-species syndecan family members did not efficiently compete with these interactions.	bind
24791	1	6643	5	13	NULL	NULL	NULL	L4 protein	GP		bind			region joining alpha3 and alpha2 helices		23S rRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_49_6_935_s_77	12039885	14 This region is located in a segment of the L4 protein joining two alpha-helices, designated alpha3 and alpha2, which is essential for the binding of this protein to 23S rRNA.	bind
31143	1	6643	6	13	NULL	NULL	NULL	L4 protein	GP		bind			region joining alpha3 and alpha2 helices		23S rRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_49_6_935_s_77	12039885	14 This region is located in a segment of the L4 protein joining two alpha-helices, designated alpha3 and alpha2, which is essential for the binding of this protein to 23S rRNA.	bind
21557	1	6645	5	13	NULL	NULL	NULL	HEB	GP		interacts with		possibly			SRF	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_8_840_s_159	12663487	14 Using EMSAs, we investigated the possibility that HEB or E2-2 interacted with SRF (through the formation of a stable ternary complex on a CArG probe or E-box probe) or enhanced SRF binding to a CArG probe.	bind
21558	2	6645	5	13	NULL	NULL	NULL	E2-2	GP		interacts with		possibly			SRF	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_8_840_s_159	12663487	14 Using EMSAs, we investigated the possibility that HEB or E2-2 interacted with SRF (through the formation of a stable ternary complex on a CArG probe or E-box probe) or enhanced SRF binding to a CArG probe.	bind
21559	3	6645	5	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_8_840_s_159	12663487	14 Using EMSAs, we investigated the possibility that HEB or E2-2 interacted with SRF (through the formation of a stable ternary complex on a CArG probe or E-box probe) or enhanced SRF binding to a CArG probe.	bind
21565	5	6645	5	13	NULL	NULL	NULL	statement 1	Process		occurs through					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_8_840_s_159	12663487	14 Using EMSAs, we investigated the possibility that HEB or E2-2 interacted with SRF (through the formation of a stable ternary complex on a CArG probe or E-box probe) or enhanced SRF binding to a CArG probe.	bind
21567	7	6645	5	13	NULL	NULL	NULL	statement 1	Process		occurs through					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_8_840_s_159	12663487	14 Using EMSAs, we investigated the possibility that HEB or E2-2 interacted with SRF (through the formation of a stable ternary complex on a CArG probe or E-box probe) or enhanced SRF binding to a CArG probe.	bind
21568	8	6645	5	13	NULL	NULL	NULL	statement 5	Process		is an alternative to					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_8_840_s_159	12663487	14 Using EMSAs, we investigated the possibility that HEB or E2-2 interacted with SRF (through the formation of a stable ternary complex on a CArG probe or E-box probe) or enhanced SRF binding to a CArG probe.	bind
21570	9	6645	5	13	NULL	NULL	NULL	statement 2	Process		occurs through					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_8_840_s_159	12663487	14 Using EMSAs, we investigated the possibility that HEB or E2-2 interacted with SRF (through the formation of a stable ternary complex on a CArG probe or E-box probe) or enhanced SRF binding to a CArG probe.	bind
21577	10	6645	5	13	NULL	NULL	NULL	statement 2	Process		occurs through					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_8_840_s_159	12663487	14 Using EMSAs, we investigated the possibility that HEB or E2-2 interacted with SRF (through the formation of a stable ternary complex on a CArG probe or E-box probe) or enhanced SRF binding to a CArG probe.	bind
21578	11	6645	5	13	NULL	NULL	NULL	statement 9	Process		is an alternative to					statement 10	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_8_840_s_159	12663487	14 Using EMSAs, we investigated the possibility that HEB or E2-2 interacted with SRF (through the formation of a stable ternary complex on a CArG probe or E-box probe) or enhanced SRF binding to a CArG probe.	bind
21579	12	6645	5	13	NULL	NULL	NULL	SRF	GP		bind					CArG probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_8_840_s_159	12663487	14 Using EMSAs, we investigated the possibility that HEB or E2-2 interacted with SRF (through the formation of a stable ternary complex on a CArG probe or E-box probe) or enhanced SRF binding to a CArG probe.	bind
30342	4	6645	5	13	NULL	NULL	NULL	ternary complex	GP	stable	forms on					CArG probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_8_840_s_159	12663487	14 Using EMSAs, we investigated the possibility that HEB or E2-2 interacted with SRF (through the formation of a stable ternary complex on a CArG probe or E-box probe) or enhanced SRF binding to a CArG probe.	bind
30343	6	6645	5	13	NULL	NULL	NULL	ternary complex	GP	stable	forms on					E-box probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_8_840_s_159	12663487	14 Using EMSAs, we investigated the possibility that HEB or E2-2 interacted with SRF (through the formation of a stable ternary complex on a CArG probe or E-box probe) or enhanced SRF binding to a CArG probe.	bind
18944	1	6645	6	13	NULL	NULL	NULL	HEB	GP		interacts with					SRF	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_8_840_s_159	12663487	14 Using EMSAs, we investigated the possibility that HEB or E2-2 interacted with SRF (through the formation of a stable ternary complex on a CArG probe or E-box probe) or enhanced SRF binding to a CArG probe.	bind
18945	2	6645	6	13	NULL	NULL	NULL	E2-2	GP		interacts with					SRF	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_8_840_s_159	12663487	14 Using EMSAs, we investigated the possibility that HEB or E2-2 interacted with SRF (through the formation of a stable ternary complex on a CArG probe or E-box probe) or enhanced SRF binding to a CArG probe.	bind
18946	3	6645	6	13	NULL	NULL	NULL	SRF	GP		bind									CArG probe	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_8_840_s_159	12663487	14 Using EMSAs, we investigated the possibility that HEB or E2-2 interacted with SRF (through the formation of a stable ternary complex on a CArG probe or E-box probe) or enhanced SRF binding to a CArG probe.	bind
19047	4	6645	6	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_8_840_s_159	12663487	14 Using EMSAs, we investigated the possibility that HEB or E2-2 interacted with SRF (through the formation of a stable ternary complex on a CArG probe or E-box probe) or enhanced SRF binding to a CArG probe.	bind
19048	6	6645	6	13	NULL	NULL	NULL	ternary complex	GP	stable	forms on					E-box probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_8_840_s_159	12663487	14 Using EMSAs, we investigated the possibility that HEB or E2-2 interacted with SRF (through the formation of a stable ternary complex on a CArG probe or E-box probe) or enhanced SRF binding to a CArG probe.	bind
19049	7	6645	6	13	NULL	NULL	NULL	statement 1	Process		occurs through					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_8_840_s_159	12663487	14 Using EMSAs, we investigated the possibility that HEB or E2-2 interacted with SRF (through the formation of a stable ternary complex on a CArG probe or E-box probe) or enhanced SRF binding to a CArG probe.	bind
30461	5	6645	6	13	NULL	NULL	NULL	ternary complex	GP	stable	forms on					CArG probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_8_840_s_159	12663487	14 Using EMSAs, we investigated the possibility that HEB or E2-2 interacted with SRF (through the formation of a stable ternary complex on a CArG probe or E-box probe) or enhanced SRF binding to a CArG probe.	bind
30462	8	6645	6	13	NULL	NULL	NULL	statement 1	Process		occurs through					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_8_840_s_159	12663487	14 Using EMSAs, we investigated the possibility that HEB or E2-2 interacted with SRF (through the formation of a stable ternary complex on a CArG probe or E-box probe) or enhanced SRF binding to a CArG probe.	bind
30463	9	6645	6	13	NULL	NULL	NULL	statement 2	Process		occurs through					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_8_840_s_159	12663487	14 Using EMSAs, we investigated the possibility that HEB or E2-2 interacted with SRF (through the formation of a stable ternary complex on a CArG probe or E-box probe) or enhanced SRF binding to a CArG probe.	bind
56221	10	6645	6	13	NULL	NULL	NULL	statement 2	Process		occurs through					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_8_840_s_159	12663487	14 Using EMSAs, we investigated the possibility that HEB or E2-2 interacted with SRF (through the formation of a stable ternary complex on a CArG probe or E-box probe) or enhanced SRF binding to a CArG probe.	bind
56222	11	6645	6	13	NULL	NULL	NULL	statement 7	Process		is an alternative to					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_8_840_s_159	12663487	14 Using EMSAs, we investigated the possibility that HEB or E2-2 interacted with SRF (through the formation of a stable ternary complex on a CArG probe or E-box probe) or enhanced SRF binding to a CArG probe.	bind
56223	12	6645	6	13	NULL	NULL	NULL	statement 9	Process		is an alternative to					statement 10	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_8_840_s_159	12663487	14 Using EMSAs, we investigated the possibility that HEB or E2-2 interacted with SRF (through the formation of a stable ternary complex on a CArG probe or E-box probe) or enhanced SRF binding to a CArG probe.	bind
21618	1	6646	5	13	NULL	NULL	NULL	Dpp	GP		is a type of					typical ABC transporter	GP				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_51_4_821_s_32	12654735	14, 17 Dpp and Opp are typical ABC transporters energized by ATP; each comprises four membrane proteins plus a periplasmic peptide binding protein DppA or OppA, respectively.	bind
21619	2	6646	5	13	NULL	NULL	NULL	statement 1	Process		is energized by					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_51_4_821_s_32	12654735	14, 17 Dpp and Opp are typical ABC transporters energized by ATP; each comprises four membrane proteins plus a periplasmic peptide binding protein DppA or OppA, respectively.	bind
21620	3	6646	5	13	NULL	NULL	NULL	Opp	GP		is a type of					typical ABC transporter	GP				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_51_4_821_s_32	12654735	14, 17 Dpp and Opp are typical ABC transporters energized by ATP; each comprises four membrane proteins plus a periplasmic peptide binding protein DppA or OppA, respectively.	bind
21621	4	6646	5	13	NULL	NULL	NULL	statement 3	Process		is energized by					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_51_4_821_s_32	12654735	14, 17 Dpp and Opp are typical ABC transporters energized by ATP; each comprises four membrane proteins plus a periplasmic peptide binding protein DppA or OppA, respectively.	bind
21623	5	6646	5	13	NULL	NULL	NULL	Dpp	GP		comprises					four membrane proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_51_4_821_s_32	12654735	14, 17 Dpp and Opp are typical ABC transporters energized by ATP; each comprises four membrane proteins plus a periplasmic peptide binding protein DppA or OppA, respectively.	bind
21624	6	6646	5	13	NULL	NULL	NULL	Dpp	GP		comprises					DppA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_51_4_821_s_32	12654735	14, 17 Dpp and Opp are typical ABC transporters energized by ATP; each comprises four membrane proteins plus a periplasmic peptide binding protein DppA or OppA, respectively.	bind
21625	7	6646	5	13	NULL	NULL	NULL	DppA	GP		is a type of					periplasmic peptide binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_51_4_821_s_32	12654735	14, 17 Dpp and Opp are typical ABC transporters energized by ATP; each comprises four membrane proteins plus a periplasmic peptide binding protein DppA or OppA, respectively.	bind
21626	8	6646	5	13	NULL	NULL	NULL	Opp	GP		comprises					four membrane proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_51_4_821_s_32	12654735	14, 17 Dpp and Opp are typical ABC transporters energized by ATP; each comprises four membrane proteins plus a periplasmic peptide binding protein DppA or OppA, respectively.	bind
21627	9	6646	5	13	NULL	NULL	NULL	Opp	GP		comprises					OppA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_51_4_821_s_32	12654735	14, 17 Dpp and Opp are typical ABC transporters energized by ATP; each comprises four membrane proteins plus a periplasmic peptide binding protein DppA or OppA, respectively.	bind
21628	10	6646	5	13	NULL	NULL	NULL	OppA	GP		is a type of					periplasmic peptide binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_51_4_821_s_32	12654735	14, 17 Dpp and Opp are typical ABC transporters energized by ATP; each comprises four membrane proteins plus a periplasmic peptide binding protein DppA or OppA, respectively.	bind
56228	11	6646	5	13	NULL	NULL	NULL	statement 5	Process		occur simultaneous with					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_51_4_821_s_32	12654735	14, 17 Dpp and Opp are typical ABC transporters energized by ATP; each comprises four membrane proteins plus a periplasmic peptide binding protein DppA or OppA, respectively.	bind
56229	12	6646	5	13	NULL	NULL	NULL	statement 8	Process		occur simultaneous with					statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_51_4_821_s_32	12654735	14, 17 Dpp and Opp are typical ABC transporters energized by ATP; each comprises four membrane proteins plus a periplasmic peptide binding protein DppA or OppA, respectively.	bind
18749	1	6646	6	13	NULL	NULL	NULL	Dpp	GP		is a type of					ABC transporter	GP				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_51_4_821_s_32	12654735	14, 17 Dpp and Opp are typical ABC transporters energized by ATP; each comprises four membrane proteins plus a periplasmic peptide binding protein DppA or OppA, respectively.	bind
18750	2	6646	6	13	NULL	NULL	NULL	statement 1	Process		is energized by					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_51_4_821_s_32	12654735	14, 17 Dpp and Opp are typical ABC transporters energized by ATP; each comprises four membrane proteins plus a periplasmic peptide binding protein DppA or OppA, respectively.	bind
18751	3	6646	6	13	NULL	NULL	NULL	Opp	GP		is a type of					ABC transporter	GP				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_51_4_821_s_32	12654735	14, 17 Dpp and Opp are typical ABC transporters energized by ATP; each comprises four membrane proteins plus a periplasmic peptide binding protein DppA or OppA, respectively.	bind
18752	4	6646	6	13	NULL	NULL	NULL	statement 3	Process		is energized by					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_51_4_821_s_32	12654735	14, 17 Dpp and Opp are typical ABC transporters energized by ATP; each comprises four membrane proteins plus a periplasmic peptide binding protein DppA or OppA, respectively.	bind
30464	5	6646	6	13	NULL	NULL	NULL	Dpp	GP		comprises of					four membrane proteins 	GP				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_51_4_821_s_32	12654735	14, 17 Dpp and Opp are typical ABC transporters energized by ATP; each comprises four membrane proteins plus a periplasmic peptide binding protein DppA or OppA, respectively.	bind
30465	6	6646	6	13	NULL	NULL	NULL	DppA	GP		is a type of					periplasmic peptide binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_51_4_821_s_32	12654735	14, 17 Dpp and Opp are typical ABC transporters energized by ATP; each comprises four membrane proteins plus a periplasmic peptide binding protein DppA or OppA, respectively.	bind
30466	7	6646	6	13	NULL	NULL	NULL	Opp	GP		comprises of					four membrane proteins 	GP				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_51_4_821_s_32	12654735	14, 17 Dpp and Opp are typical ABC transporters energized by ATP; each comprises four membrane proteins plus a periplasmic peptide binding protein DppA or OppA, respectively.	bind
30467	8	6646	6	13	NULL	NULL	NULL	OppA	GP		is a type of					periplasmic peptide binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_51_4_821_s_32	12654735	14, 17 Dpp and Opp are typical ABC transporters energized by ATP; each comprises four membrane proteins plus a periplasmic peptide binding protein DppA or OppA, respectively.	bind
56224	9	6646	6	13	NULL	NULL	NULL	Dpp	GP		comprise of					DppA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_51_4_821_s_32	12654735	14, 17 Dpp and Opp are typical ABC transporters energized by ATP; each comprises four membrane proteins plus a periplasmic peptide binding protein DppA or OppA, respectively.	bind
56225	10	6646	6	13	NULL	NULL	NULL	Opp	GP		comprise of					OppA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_51_4_821_s_32	12654735	14, 17 Dpp and Opp are typical ABC transporters energized by ATP; each comprises four membrane proteins plus a periplasmic peptide binding protein DppA or OppA, respectively.	bind
56226	11	6646	6	13	NULL	NULL	NULL	statement 5	Process		occur simultaneous with					statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_51_4_821_s_32	12654735	14, 17 Dpp and Opp are typical ABC transporters energized by ATP; each comprises four membrane proteins plus a periplasmic peptide binding protein DppA or OppA, respectively.	bind
56227	12	6646	6	13	NULL	NULL	NULL	statement 7	Process		occur simultaneous with					statement 10	Process				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_51_4_821_s_32	12654735	14, 17 Dpp and Opp are typical ABC transporters energized by ATP; each comprises four membrane proteins plus a periplasmic peptide binding protein DppA or OppA, respectively.	bind
21630	1	6647	5	13	NULL	NULL	NULL	myosin light chain phosphatase	GP		is target of		major			Rho-kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_13_1545_s_70	11927519	14, 17 In that model, it was shown that inactivation of the myosin-binding subunit of myosin light chain phosphatase, which is a major target protein of Rho-kinase, was a primary mechanism whereby fasudil or Y27632 prevented coronary artery spasm.	bind
21631	2	6647	5	13	NULL	NULL	NULL	fasudil	Chemical		prevents					coronary artery spasm	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_13_1545_s_70	11927519	14, 17 In that model, it was shown that inactivation of the myosin-binding subunit of myosin light chain phosphatase, which is a major target protein of Rho-kinase, was a primary mechanism whereby fasudil or Y27632 prevented coronary artery spasm.	bind
21632	3	6647	5	13	NULL	NULL	NULL				prevents			Y27632		coronary artery spasm	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_13_1545_s_70	11927519	14, 17 In that model, it was shown that inactivation of the myosin-binding subunit of myosin light chain phosphatase, which is a major target protein of Rho-kinase, was a primary mechanism whereby fasudil or Y27632 prevented coronary artery spasm.	bind
21633	4	6647	5	13	NULL	NULL	NULL	myosin-binding subunit 	GP		is a subunit of					myosin light chain phosphatase	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_13_1545_s_70	11927519	14, 17 In that model, it was shown that inactivation of the myosin-binding subunit of myosin light chain phosphatase, which is a major target protein of Rho-kinase, was a primary mechanism whereby fasudil or Y27632 prevented coronary artery spasm.	bind
21635	5	6647	5	13	NULL	NULL	NULL	statement 4	Process	inactivation of	mechanism for		primary			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_13_1545_s_70	11927519	14, 17 In that model, it was shown that inactivation of the myosin-binding subunit of myosin light chain phosphatase, which is a major target protein of Rho-kinase, was a primary mechanism whereby fasudil or Y27632 prevented coronary artery spasm.	bind
21636	6	6647	5	13	NULL	NULL	NULL	statement 4	Process	inactivation of	mechanism for		primary			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_13_1545_s_70	11927519	14, 17 In that model, it was shown that inactivation of the myosin-binding subunit of myosin light chain phosphatase, which is a major target protein of Rho-kinase, was a primary mechanism whereby fasudil or Y27632 prevented coronary artery spasm.	bind
18753	1	6647	6	13	NULL	NULL	NULL	fasudil	Chemical		prevents					coronary artery spasm	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_13_1545_s_70	11927519	14, 17 In that model, it was shown that inactivation of the myosin-binding subunit of myosin light chain phosphatase, which is a major target protein of Rho-kinase, was a primary mechanism whereby fasudil or Y27632 prevented coronary artery spasm.	bind
18754	2	6647	6	13	NULL	NULL	NULL				prevents			Y27632		coronary artery spasm	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_13_1545_s_70	11927519	14, 17 In that model, it was shown that inactivation of the myosin-binding subunit of myosin light chain phosphatase, which is a major target protein of Rho-kinase, was a primary mechanism whereby fasudil or Y27632 prevented coronary artery spasm.	bind
18755	4	6647	6	13	NULL	NULL	NULL	statement 3	Process	inactivation of	mechanism for		primary			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_13_1545_s_70	11927519	14, 17 In that model, it was shown that inactivation of the myosin-binding subunit of myosin light chain phosphatase, which is a major target protein of Rho-kinase, was a primary mechanism whereby fasudil or Y27632 prevented coronary artery spasm.	bind
18756	5	6647	6	13	NULL	NULL	NULL	statement 3	Process	inactivation of	mechanism for		primary			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_13_1545_s_70	11927519	14, 17 In that model, it was shown that inactivation of the myosin-binding subunit of myosin light chain phosphatase, which is a major target protein of Rho-kinase, was a primary mechanism whereby fasudil or Y27632 prevented coronary artery spasm.	bind
56230	3	6647	6	13	NULL	NULL	NULL	myosin-binding subunit	GP		is a subunit of					 myosin light chain phosphatase	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_13_1545_s_70	11927519	14, 17 In that model, it was shown that inactivation of the myosin-binding subunit of myosin light chain phosphatase, which is a major target protein of Rho-kinase, was a primary mechanism whereby fasudil or Y27632 prevented coronary artery spasm.	bind
56231	6	6647	6	13	NULL	NULL	NULL	 myosin light chain phosphatase	GP		target protein of					Rho-kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_13_1545_s_70	11927519	14, 17 In that model, it was shown that inactivation of the myosin-binding subunit of myosin light chain phosphatase, which is a major target protein of Rho-kinase, was a primary mechanism whereby fasudil or Y27632 prevented coronary artery spasm.	bind
21637	1	6648	5	13	NULL	NULL	NULL	CXCR2	GP		bind					Gro-alpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_3_753_s_284	10487833	14, 53 The CXCR2 also binds another member of the CXC chemokine superfamily, the chemokine growth- related oncogene alpha (synonymous with melanoma growth-stimulating activity) Gro-alpha, which is also known to act as an autocrine growth factor for melanoma.	bind
21654	2	6648	5	13	NULL	NULL	NULL	Gro-alpha	GP		is					chemokine growth- related oncogene alpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_3_753_s_284	10487833	14, 53 The CXCR2 also binds another member of the CXC chemokine superfamily, the chemokine growth- related oncogene alpha (synonymous with melanoma growth-stimulating activity) Gro-alpha, which is also known to act as an autocrine growth factor for melanoma.	bind
21655	3	6648	5	13	NULL	NULL	NULL	chemokine growth- related oncogene alpha	GP		is synonymous with					melanoma growth-stimulating activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_3_753_s_284	10487833	14, 53 The CXCR2 also binds another member of the CXC chemokine superfamily, the chemokine growth- related oncogene alpha (synonymous with melanoma growth-stimulating activity) Gro-alpha, which is also known to act as an autocrine growth factor for melanoma.	bind
21656	4	6648	5	13	NULL	NULL	NULL	Gro-alpha	GP		acts as					autocrine growth factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_3_753_s_284	10487833	14, 53 The CXCR2 also binds another member of the CXC chemokine superfamily, the chemokine growth- related oncogene alpha (synonymous with melanoma growth-stimulating activity) Gro-alpha, which is also known to act as an autocrine growth factor for melanoma.	bind
44668	5	6648	5	13	NULL	NULL	NULL	statement 4	Process		occurs for					melanoma	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_3_753_s_284	10487833	14, 53 The CXCR2 also binds another member of the CXC chemokine superfamily, the chemokine growth- related oncogene alpha (synonymous with melanoma growth-stimulating activity) Gro-alpha, which is also known to act as an autocrine growth factor for melanoma.	bind
18757	1	6648	6	13	NULL	NULL	NULL	CXCR2	GP		bind					Gro-alpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_3_753_s_284	10487833	14, 53 The CXCR2 also binds another member of the CXC chemokine superfamily, the chemokine growth- related oncogene alpha (synonymous with melanoma growth-stimulating activity) Gro-alpha, which is also known to act as an autocrine growth factor for melanoma.	bind
18758	2	6648	6	13	NULL	NULL	NULL	Gro-alpha	GP		is					chemokine growth- related oncogene alpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_3_753_s_284	10487833	14, 53 The CXCR2 also binds another member of the CXC chemokine superfamily, the chemokine growth- related oncogene alpha (synonymous with melanoma growth-stimulating activity) Gro-alpha, which is also known to act as an autocrine growth factor for melanoma.	bind
18759	3	6648	6	13	NULL	NULL	NULL	Gro-alpha	GP		is synonymous with					melanoma growth-stimulating activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_3_753_s_284	10487833	14, 53 The CXCR2 also binds another member of the CXC chemokine superfamily, the chemokine growth- related oncogene alpha (synonymous with melanoma growth-stimulating activity) Gro-alpha, which is also known to act as an autocrine growth factor for melanoma.	bind
18760	4	6648	6	13	NULL	NULL	NULL	Gro-alpha	GP		acts as an					autocrine growth factor 	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_3_753_s_284	10487833	14, 53 The CXCR2 also binds another member of the CXC chemokine superfamily, the chemokine growth- related oncogene alpha (synonymous with melanoma growth-stimulating activity) Gro-alpha, which is also known to act as an autocrine growth factor for melanoma.	bind
56232	5	6648	6	13	NULL	NULL	NULL	statement 4	Process		occurs for					melanoma	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_3_753_s_284	10487833	14, 53 The CXCR2 also binds another member of the CXC chemokine superfamily, the chemokine growth- related oncogene alpha (synonymous with melanoma growth-stimulating activity) Gro-alpha, which is also known to act as an autocrine growth factor for melanoma.	bind
21657	1	6649	5	13	NULL	NULL	NULL	GTP	Chemical		bind		readily			tTG	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_10_1153_s_27	12702643	14,15  Both GTP and GDP readily bind tTG. 16 Distinct GTP binding and TG domains have been identified within Gh/tTG, 17 and the latter function may be negatively regulated by GTP binding.	bind
21658	2	6649	5	13	NULL	NULL	NULL	GDP	Chemical		bind		readily			tTG	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_10_1153_s_27	12702643	14,15  Both GTP and GDP readily bind tTG. 16 Distinct GTP binding and TG domains have been identified within Gh/tTG, 17 and the latter function may be negatively regulated by GTP binding.	bind
21659	3	6649	5	13	NULL	NULL	NULL	Gh/tTG	GP		contains							distinct	GTP binding domain		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_10_1153_s_27	12702643	14,15  Both GTP and GDP readily bind tTG. 16 Distinct GTP binding and TG domains have been identified within Gh/tTG, 17 and the latter function may be negatively regulated by GTP binding.	bind
21660	4	6649	5	13	NULL	NULL	NULL	Gh/tTG	GP		contains							distinct	TG domains		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_10_1153_s_27	12702643	14,15  Both GTP and GDP readily bind tTG. 16 Distinct GTP binding and TG domains have been identified within Gh/tTG, 17 and the latter function may be negatively regulated by GTP binding.	bind
18761	1	6649	6	13	NULL	NULL	NULL	GTP	Chemical		bind					tTG	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_10_1153_s_27	12702643	14,15  Both GTP and GDP readily bind tTG. 16 Distinct GTP binding and TG domains have been identified within Gh/tTG, 17 and the latter function may be negatively regulated by GTP binding.	bind
18762	2	6649	6	13	NULL	NULL	NULL	GDP	Chemical		bind					tTG	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_10_1153_s_27	12702643	14,15  Both GTP and GDP readily bind tTG. 16 Distinct GTP binding and TG domains have been identified within Gh/tTG, 17 and the latter function may be negatively regulated by GTP binding.	bind
30468	3	6649	6	13	NULL	NULL	NULL	Gh/tTG	GP		contain								GTP binding domain		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_10_1153_s_27	12702643	14,15  Both GTP and GDP readily bind tTG. 16 Distinct GTP binding and TG domains have been identified within Gh/tTG, 17 and the latter function may be negatively regulated by GTP binding.	bind
30469	4	6649	6	13	NULL	NULL	NULL	Gh/tTG	GP		contain								TG domain		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_10_1153_s_27	12702643	14,15  Both GTP and GDP readily bind tTG. 16 Distinct GTP binding and TG domains have been identified within Gh/tTG, 17 and the latter function may be negatively regulated by GTP binding.	bind
21661	1	6650	5	13	NULL	NULL	NULL	SRF	GP		bind									CArG elements (CC (A/T) 6-GG motif)	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_378_s_163	16397143	14,15,21,22    It activates transcription of a large subset of SMC marker genes by binding of SRF to CArG elements (CC (A/T) 6-GG motif) found in the promoters of these genes.	bind
21662	2	6650	5	13	NULL	NULL	NULL	SMC marker genes	GP	transcription of	is activated by					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_378_s_163	16397143	14,15,21,22    It activates transcription of a large subset of SMC marker genes by binding of SRF to CArG elements (CC (A/T) 6-GG motif) found in the promoters of these genes.	bind
18763	1	6650	6	13	NULL	NULL	NULL	SRF	GP		bind									CArG element	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_378_s_163	16397143	14,15,21,22    It activates transcription of a large subset of SMC marker genes by binding of SRF to CArG elements (CC (A/T) 6-GG motif) found in the promoters of these genes.	bind
31148	2	6650	6	13	NULL	NULL	NULL	statement 1	Process		activates					 SMC marker genes	GP	transcription of;;large subset of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_378_s_163	16397143	14,15,21,22    It activates transcription of a large subset of SMC marker genes by binding of SRF to CArG elements (CC (A/T) 6-GG motif) found in the promoters of these genes.	bind
21663	1	6651	5	13	NULL	NULL	NULL	Ear2	GP		bind					T3R	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_9_1033_s_210	12690040	14,17  Studies of T3R function suggest that Ear2 binds to T3R, preventing its binding to the TRE. 16 Ear2 is a member of COUP-TF family.	bind
21664	2	6651	5	13	NULL	NULL	NULL	T3R	GP		bind									TRE	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_9_1033_s_210	12690040	14,17  Studies of T3R function suggest that Ear2 binds to T3R, preventing its binding to the TRE. 16 Ear2 is a member of COUP-TF family.	bind
21665	3	6651	5	13	NULL	NULL	NULL	statement 1	Process		prevents					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_9_1033_s_210	12690040	14,17  Studies of T3R function suggest that Ear2 binds to T3R, preventing its binding to the TRE. 16 Ear2 is a member of COUP-TF family.	bind
21666	4	6651	5	13	NULL	NULL	NULL	Ear2	GP		is a member of					COUP-TF family	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_9_1033_s_210	12690040	14,17  Studies of T3R function suggest that Ear2 binds to T3R, preventing its binding to the TRE. 16 Ear2 is a member of COUP-TF family.	bind
18764	1	6651	6	13	NULL	NULL	NULL	Ear2	GP		bind					T3R	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_9_1033_s_210	12690040	14,17  Studies of T3R function suggest that Ear2 binds to T3R, preventing its binding to the TRE. 16 Ear2 is a member of COUP-TF family.	bind
18765	2	6651	6	13	NULL	NULL	NULL	T3R	GP		bind									TRE	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_9_1033_s_210	12690040	14,17  Studies of T3R function suggest that Ear2 binds to T3R, preventing its binding to the TRE. 16 Ear2 is a member of COUP-TF family.	bind
18766	3	6651	6	13	NULL	NULL	NULL	statement 1	Process		prevents					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_9_1033_s_210	12690040	14,17  Studies of T3R function suggest that Ear2 binds to T3R, preventing its binding to the TRE. 16 Ear2 is a member of COUP-TF family.	bind
18767	4	6651	6	13	NULL	NULL	NULL	Ear2	GP		is a member of					COUP-TF family	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_9_1033_s_210	12690040	14,17  Studies of T3R function suggest that Ear2 binds to T3R, preventing its binding to the TRE. 16 Ear2 is a member of COUP-TF family.	bind
21667	1	6652	5	13	NULL	NULL	NULL	14-3-3 zeta	GP		bind			amphipathic groove		Raf peptide	GP	phosphorylated			NULL		NULL	NULL	NULL	NULL	gw70_annurevplantbiol_50_0_277_s_671	null	14-3-3  zeta binds a phosphorylated Raf peptide and an unphosphorylated peptide via its conserved  amphipathic groove.	bind
21669	2	6652	5	13	NULL	NULL	NULL	14-3-3 zeta	GP		bind			amphipathic groove		peptide	GP	unphosphorylated			NULL		NULL	NULL	NULL	NULL	gw70_annurevplantbiol_50_0_277_s_671	null	14-3-3  zeta binds a phosphorylated Raf peptide and an unphosphorylated peptide via its conserved  amphipathic groove.	bind
18768	1	6652	6	13	NULL	NULL	NULL	14-3-3 zeta	GP		bind			amphipathic groove		Raf peptide	GP	phosphorylated			NULL		NULL	NULL	NULL	NULL	gw70_annurevplantbiol_50_0_277_s_671	null	14-3-3  zeta binds a phosphorylated Raf peptide and an unphosphorylated peptide via its conserved  amphipathic groove.	bind
18769	2	6652	6	13	NULL	NULL	NULL	14-3-3 zeta	GP		bind			amphipathic groove		peptide	GP	unphosphorylated			NULL		NULL	NULL	NULL	NULL	gw70_annurevplantbiol_50_0_277_s_671	null	14-3-3  zeta binds a phosphorylated Raf peptide and an unphosphorylated peptide via its conserved  amphipathic groove.	bind
21671	1	6653	5	13	NULL	NULL	NULL	14-3-3	GP		bind					tau	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_18392_s_277	14970201	14-3-3 and tubulin share a common binding site on tau, and their binding to tau is mutually exclusive ( ), suggesting that 14-3-3 may regulate binding of tau to microtubules.	bind
21672	2	6653	5	13	NULL	NULL	NULL	tubulin	GP		bind					tau	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_18392_s_277	14970201	14-3-3 and tubulin share a common binding site on tau, and their binding to tau is mutually exclusive ( ), suggesting that 14-3-3 may regulate binding of tau to microtubules.	bind
21673	3	6653	5	13	NULL	NULL	NULL	14-3-3	GP	binding site of	share with					tubulin	GP	binding site of			NULL	 Tau	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_18392_s_277	14970201	14-3-3 and tubulin share a common binding site on tau, and their binding to tau is mutually exclusive ( ), suggesting that 14-3-3 may regulate binding of tau to microtubules.	bind
21674	4	6653	5	13	NULL	NULL	NULL	statement 1	Process		is mutually exclusive to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_18392_s_277	14970201	14-3-3 and tubulin share a common binding site on tau, and their binding to tau is mutually exclusive ( ), suggesting that 14-3-3 may regulate binding of tau to microtubules.	bind
21675	5	6653	5	13	NULL	NULL	NULL	tau	GP		bind					microtubules	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_18392_s_277	14970201	14-3-3 and tubulin share a common binding site on tau, and their binding to tau is mutually exclusive ( ), suggesting that 14-3-3 may regulate binding of tau to microtubules.	bind
21676	6	6653	5	13	NULL	NULL	NULL	14-3-3	GP		regulates		may			statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_18392_s_277	14970201	14-3-3 and tubulin share a common binding site on tau, and their binding to tau is mutually exclusive ( ), suggesting that 14-3-3 may regulate binding of tau to microtubules.	bind
21677	7	6653	5	13	NULL	NULL	NULL	statement 4	Process		suggests					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_18392_s_277	14970201	14-3-3 and tubulin share a common binding site on tau, and their binding to tau is mutually exclusive ( ), suggesting that 14-3-3 may regulate binding of tau to microtubules.	bind
18770	1	6653	6	NULL	NULL	0	NULL	14-3-3	NULL		bind	NULL				tau	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_18_18392_s_277	14970201	14-3-3 and tubulin share a common binding site on tau, and their binding to tau is mutually exclusive ( ), suggesting that 14-3-3 may regulate binding of tau to microtubules.	bind
18771	2	6653	6	NULL	NULL	0	NULL	tubulin	NULL		bind	NULL				tau	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_18_18392_s_277	14970201	14-3-3 and tubulin share a common binding site on tau, and their binding to tau is mutually exclusive ( ), suggesting that 14-3-3 may regulate binding of tau to microtubules.	bind
18772	3	6653	6	NULL	NULL	0	NULL	statement 1	NULL		is independent of	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_18_18392_s_277	14970201	14-3-3 and tubulin share a common binding site on tau, and their binding to tau is mutually exclusive ( ), suggesting that 14-3-3 may regulate binding of tau to microtubules.	bind
18773	4	6653	6	NULL	NULL	0	NULL	tau	NULL		bind	NULL				microtubules	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_18_18392_s_277	14970201	14-3-3 and tubulin share a common binding site on tau, and their binding to tau is mutually exclusive ( ), suggesting that 14-3-3 may regulate binding of tau to microtubules.	bind
18774	5	6653	6	NULL	NULL	0	NULL	14-3-3	NULL		regulate	NULL	may			statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_18_18392_s_277	14970201	14-3-3 and tubulin share a common binding site on tau, and their binding to tau is mutually exclusive ( ), suggesting that 14-3-3 may regulate binding of tau to microtubules.	bind
56308	6	6653	6	10	NULL	0	NULL	14-3-3		binding site of	share with					tubulin		binding site of			NULL	Tau	0	NULL	NULL	NULL	gw70_jbiolchem_279_18_18392_s_277	14970201	14-3-3 and tubulin share a common binding site on tau, and their binding to tau is mutually exclusive ( ), suggesting that 14-3-3 may regulate binding of tau to microtubules.	bind
56309	7	6653	6	10	NULL	0	NULL	statement 3			suggest					statement 5					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_18_18392_s_277	14970201	14-3-3 and tubulin share a common binding site on tau, and their binding to tau is mutually exclusive ( ), suggesting that 14-3-3 may regulate binding of tau to microtubules.	bind
21678	1	6659	5	13	NULL	NULL	NULL	14-3-3 zeta	GP		bind					Bcr	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_46_28882_s_36	9360956	14-3-3 zeta also binds to Bcr, but is not phosphorylated ( 19).	bind
21679	2	6659	5	13	NULL	NULL	NULL	14-3-3 zeta	GP		does not undergo					phosphorylation	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_46_28882_s_36	9360956	14-3-3 zeta also binds to Bcr, but is not phosphorylated ( 19).	bind
18775	1	6659	6	NULL	NULL	0	NULL	14-3-3 zeta	NULL	unphosphorylated	bind	NULL				Bcr	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_46_28882_s_36	9360956	14-3-3 zeta also binds to Bcr, but is not phosphorylated ( 19).	bind
21680	1	6660	5	13	NULL	NULL	NULL	Nedd4-2	GP		bind					alpha-ENaC	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_24_16323_s_197	16613846	14-3-3beta knockdown reverses the aldosterone-induced decrease in Nedd4-2 binding to alpha-ENaC.	bind
21681	2	6660	5	13	NULL	NULL	NULL	aldosterone	Chemical	induction of	decreases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_24_16323_s_197	16613846	14-3-3beta knockdown reverses the aldosterone-induced decrease in Nedd4-2 binding to alpha-ENaC.	bind
21682	3	6660	5	13	NULL	NULL	NULL	14-3-3beta	GP	knockdown of	reverses					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_24_16323_s_197	16613846	14-3-3beta knockdown reverses the aldosterone-induced decrease in Nedd4-2 binding to alpha-ENaC.	bind
18776	1	6660	6	NULL	NULL	0	NULL	Nedd4-2	NULL		bind	NULL				alpha-ENaC	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_24_16323_s_197	16613846	14-3-3beta knockdown reverses the aldosterone-induced decrease in Nedd4-2 binding to alpha-ENaC.	bind
18777	2	6660	6	NULL	NULL	0	NULL	aldosterone	NULL		decreases	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_24_16323_s_197	16613846	14-3-3beta knockdown reverses the aldosterone-induced decrease in Nedd4-2 binding to alpha-ENaC.	bind
18778	3	6660	6	NULL	NULL	0	NULL	14-3-3beta	NULL	knockdown of	reverses	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_24_16323_s_197	16613846	14-3-3beta knockdown reverses the aldosterone-induced decrease in Nedd4-2 binding to alpha-ENaC.	bind
21683	1	6663	5	13	NULL	NULL	NULL	14C-ADP	Chemical		bind					platelet membranes	CellComponent	normal human			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_311	9108793	14C-ADP binding to normal human and thrombasthenic platelet membranes: study of the dissociation of the nucleotide from its receptors.	bind
21684	2	6663	5	13	NULL	NULL	NULL	14C-ADP	Chemical		bind					platelet membranes	CellComponent	thrombasthenic			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_311	9108793	14C-ADP binding to normal human and thrombasthenic platelet membranes: study of the dissociation of the nucleotide from its receptors.	bind
18779	1	6663	6	NULL	NULL	0	NULL	14C-ADP	NULL		bind	NULL				platelet membrane	NULL	normal human			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_311	9108793	14C-ADP binding to normal human and thrombasthenic platelet membranes: study of the dissociation of the nucleotide from its receptors.	bind
18780	2	6663	6	NULL	NULL	0	NULL	14C-ADP	NULL		bind	NULL				platelet membrane	NULL	thrombasthenic			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_311	9108793	14C-ADP binding to normal human and thrombasthenic platelet membranes: study of the dissociation of the nucleotide from its receptors.	bind
21685	1	6665	5	13	NULL	NULL	NULL	DpnM DNA adenine methyltransferase	GP	DpnII restriction system of Streptococcus pneumoniae	bind					S-adenosylmethionine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_7_1491_s_434	11266551	15       Tran,P.H., Korszun,Z.R., Cerritelli,S., Springhorn,S.S. and Lacks,S.A. (1998) Crystal structure of the  DpnM DNA adenine methyltransferase from the  DpnII restriction system of  Streptococcus pneumoniae bound to  S-adenosylmethionine.	bind
18781	1	6665	6	NULL	NULL	0	NULL	DpnM DNA adenine methyltransferase	NULL	streptococcus pneumoniae	bind	NULL				S-adenosylmethionine	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_7_1491_s_434	11266551	15       Tran,P.H., Korszun,Z.R., Cerritelli,S., Springhorn,S.S. and Lacks,S.A. (1998) Crystal structure of the  DpnM DNA adenine methyltransferase from the  DpnII restriction system of  Streptococcus pneumoniae bound to  S-adenosylmethionine.	bind
21686	1	6666	5	13	NULL	NULL	NULL	VEGF-C	GP		bind					VEGFR-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_7_s_23	10880369	15  A proteolytically processed form of VEGF-C can also bind to VEGFR-2, which is expressed in both blood and lymphatic vessel endothelia.	bind
21687	2	6666	5	13	NULL	NULL	NULL	VEGF-C	GP		is processed					proteolytically	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_7_s_23	10880369	15  A proteolytically processed form of VEGF-C can also bind to VEGFR-2, which is expressed in both blood and lymphatic vessel endothelia.	bind
30344	3	6666	5	13	NULL	NULL	NULL	VEGFR-2	GP		is expressed in					blood vessel endothelia	Cell				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_7_s_23	10880369	15  A proteolytically processed form of VEGF-C can also bind to VEGFR-2, which is expressed in both blood and lymphatic vessel endothelia.	bind
30345	4	6666	5	13	NULL	NULL	NULL	VEGFR-2	GP		is expressed in					lymphatic vessel endothelia	Cell				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_7_s_23	10880369	15  A proteolytically processed form of VEGF-C can also bind to VEGFR-2, which is expressed in both blood and lymphatic vessel endothelia.	bind
18782	1	6666	6	NULL	NULL	0	NULL	VEGF-C	NULL		bind	NULL				VEGFR-2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_7_s_23	10880369	15  A proteolytically processed form of VEGF-C can also bind to VEGFR-2, which is expressed in both blood and lymphatic vessel endothelia.	bind
18783	2	6666	6	10	NULL	0	NULL	VEGFR-2			expressed in					blood vessel endothelia					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_7_s_23	10880369	15  A proteolytically processed form of VEGF-C can also bind to VEGFR-2, which is expressed in both blood and lymphatic vessel endothelia.	bind
18784	3	6666	6	10	NULL	0	NULL	VEGFR-2			expressed in					lymphatic vessel endothelia					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_7_s_23	10880369	15  A proteolytically processed form of VEGF-C can also bind to VEGFR-2, which is expressed in both blood and lymphatic vessel endothelia.	bind
32786	4	6666	6	NULL	NULL	0	NULL	VEGF-C	NULL		is processed 	NULL				proteolytically	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_1_7_s_23	10880369	15  A proteolytically processed form of VEGF-C can also bind to VEGFR-2, which is expressed in both blood and lymphatic vessel endothelia.	bind
21689	1	6667	5	13	NULL	NULL	NULL	EPCR	GP		bind		specifically			protein C	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_10_3633_s_29	9396465	15  EPCR binds specifically to either protein C or APC. 15  Binding of protein C to EPCR promotes protein C activation 17  and blocks APC anticoagulant activity.	bind
21691	2	6667	5	13	NULL	NULL	NULL	EPCR	GP		bind		specifically			APC	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_10_3633_s_29	9396465	15  EPCR binds specifically to either protein C or APC. 15  Binding of protein C to EPCR promotes protein C activation 17  and blocks APC anticoagulant activity.	bind
21692	3	6667	5	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_10_3633_s_29	9396465	15  EPCR binds specifically to either protein C or APC. 15  Binding of protein C to EPCR promotes protein C activation 17  and blocks APC anticoagulant activity.	bind
21693	4	6667	5	13	NULL	NULL	NULL	statement 1	Process		promote					protein C	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_10_3633_s_29	9396465	15  EPCR binds specifically to either protein C or APC. 15  Binding of protein C to EPCR promotes protein C activation 17  and blocks APC anticoagulant activity.	bind
21694	5	6667	5	13	NULL	NULL	NULL	statement 1	Process		blocks					APC	GP	anticoagulant activity of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_10_3633_s_29	9396465	15  EPCR binds specifically to either protein C or APC. 15  Binding of protein C to EPCR promotes protein C activation 17  and blocks APC anticoagulant activity.	bind
18785	1	6667	6	NULL	NULL	0	NULL	EPCR	NULL		bind	NULL	specifically			protein C	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_10_3633_s_29	9396465	15  EPCR binds specifically to either protein C or APC. 15  Binding of protein C to EPCR promotes protein C activation 17  and blocks APC anticoagulant activity.	bind
18786	2	6667	6	NULL	NULL	0	NULL	EPCR	NULL		bind	NULL	specifically			APC	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_96_10_3633_s_29	9396465	15  EPCR binds specifically to either protein C or APC. 15  Binding of protein C to EPCR promotes protein C activation 17  and blocks APC anticoagulant activity.	bind
18787	3	6667	6	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_96_10_3633_s_29	9396465	15  EPCR binds specifically to either protein C or APC. 15  Binding of protein C to EPCR promotes protein C activation 17  and blocks APC anticoagulant activity.	bind
18788	4	6667	6	NULL	NULL	0	NULL	statement 1	NULL		promotes	NULL				protein C	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_circulation_96_10_3633_s_29	9396465	15  EPCR binds specifically to either protein C or APC. 15  Binding of protein C to EPCR promotes protein C activation 17  and blocks APC anticoagulant activity.	bind
18790	5	6667	6	10	NULL	0	NULL	statement 1			blocks					APC		anticoagulant activity of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_10_3633_s_29	9396465	15  EPCR binds specifically to either protein C or APC. 15  Binding of protein C to EPCR promotes protein C activation 17  and blocks APC anticoagulant activity.	bind
21695	1	6668	5	13	NULL	NULL	NULL	sPLA2	GP		bind					decorin	GP		core protein		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulationres_86_6_610_s_28	10746993	15  In this issue of  Circulation Research, the investigation group reports that sPLA2 can bind to both the core protein and the glycosaminoglycan chains of decorin in vitro.	bind
21696	2	6668	5	13	NULL	NULL	NULL	sPLA2	GP		bind					decorin	GP		glycosaminoglycan chains		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulationres_86_6_610_s_28	10746993	15  In this issue of  Circulation Research, the investigation group reports that sPLA2 can bind to both the core protein and the glycosaminoglycan chains of decorin in vitro.	bind
18791	1	6668	6	NULL	NULL	0	NULL	sPLA2	NULL		bind	NULL				decorin	NULL		core protein		NULL	in vitro	0	NULL	NULL	NULL	gw60_circulationres_86_6_610_s_28	10746993	15  In this issue of  Circulation Research, the investigation group reports that sPLA2 can bind to both the core protein and the glycosaminoglycan chains of decorin in vitro.	bind
18792	2	6668	6	NULL	NULL	0	NULL	sPLA2	NULL		bind	NULL				decorin	NULL		glycosaminoglycan chains		NULL	in vitro	0	NULL	NULL	NULL	gw60_circulationres_86_6_610_s_28	10746993	15  In this issue of  Circulation Research, the investigation group reports that sPLA2 can bind to both the core protein and the glycosaminoglycan chains of decorin in vitro.	bind
21697	1	6669	5	13	NULL	NULL	NULL	CTL cells	Cell		recognizes					susceptible target cell	Cell				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1805_s_23	10362805	15  In this pathway, the recognition and tight binding of a susceptible target cell by a CTL or NK cell induces the release of electron-dense cytoplasmic granules by the effector cells.	bind
21698	2	6669	5	13	NULL	NULL	NULL	NK cells	Cell		recognizes					susceptible target cell	Cell				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1805_s_23	10362805	15  In this pathway, the recognition and tight binding of a susceptible target cell by a CTL or NK cell induces the release of electron-dense cytoplasmic granules by the effector cells.	bind
21699	3	6669	5	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1805_s_23	10362805	15  In this pathway, the recognition and tight binding of a susceptible target cell by a CTL or NK cell induces the release of electron-dense cytoplasmic granules by the effector cells.	bind
21700	4	6669	5	13	NULL	NULL	NULL	CTL cells	Cell		bind		tightly			susceptible target cell	Cell				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1805_s_23	10362805	15  In this pathway, the recognition and tight binding of a susceptible target cell by a CTL or NK cell induces the release of electron-dense cytoplasmic granules by the effector cells.	bind
21701	5	6669	5	13	NULL	NULL	NULL	NK cells	Cell		bind		tightly			susceptible target cell	Cell				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1805_s_23	10362805	15  In this pathway, the recognition and tight binding of a susceptible target cell by a CTL or NK cell induces the release of electron-dense cytoplasmic granules by the effector cells.	bind
21702	6	6669	5	13	NULL	NULL	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1805_s_23	10362805	15  In this pathway, the recognition and tight binding of a susceptible target cell by a CTL or NK cell induces the release of electron-dense cytoplasmic granules by the effector cells.	bind
21704	7	6669	5	13	NULL	NULL	NULL	effector cells	Cell		release					electron-dense cytoplasmic granules	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1805_s_23	10362805	15  In this pathway, the recognition and tight binding of a susceptible target cell by a CTL or NK cell induces the release of electron-dense cytoplasmic granules by the effector cells.	bind
21706	8	6669	5	13	NULL	NULL	NULL	statement 3	Process		induces					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1805_s_23	10362805	15  In this pathway, the recognition and tight binding of a susceptible target cell by a CTL or NK cell induces the release of electron-dense cytoplasmic granules by the effector cells.	bind
21708	9	6669	5	13	NULL	NULL	NULL	statement 6	Process		induces					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1805_s_23	10362805	15  In this pathway, the recognition and tight binding of a susceptible target cell by a CTL or NK cell induces the release of electron-dense cytoplasmic granules by the effector cells.	bind
18947	1	6669	6	10	NULL	0	NULL	CTL			bind		tightly			susceptible target cell					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1805_s_23	10362805	15  In this pathway, the recognition and tight binding of a susceptible target cell by a CTL or NK cell induces the release of electron-dense cytoplasmic granules by the effector cells.	bind
18948	2	6669	6	10	NULL	0	NULL	NK cell			bind		tightly			susceptible target cell					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1805_s_23	10362805	15  In this pathway, the recognition and tight binding of a susceptible target cell by a CTL or NK cell induces the release of electron-dense cytoplasmic granules by the effector cells.	bind
18968	4	6669	6	10	NULL	0	NULL	CTL			recognizes					susceptible target cell					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1805_s_23	10362805	15  In this pathway, the recognition and tight binding of a susceptible target cell by a CTL or NK cell induces the release of electron-dense cytoplasmic granules by the effector cells.	bind
18970	5	6669	6	10	NULL	0	NULL	NK cells			recognizes					susceptible target cell					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1805_s_23	10362805	15  In this pathway, the recognition and tight binding of a susceptible target cell by a CTL or NK cell induces the release of electron-dense cytoplasmic granules by the effector cells.	bind
19050	6	6669	6	10	NULL	0	NULL	statement 1			is an alternative to					statement 2					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1805_s_23	10362805	15  In this pathway, the recognition and tight binding of a susceptible target cell by a CTL or NK cell induces the release of electron-dense cytoplasmic granules by the effector cells.	bind
56336	3	6669	6	10	NULL	0	NULL	effector cells			release					 electron-dense cytoplasmic granules					NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_6_1805_s_23	10362805	15  In this pathway, the recognition and tight binding of a susceptible target cell by a CTL or NK cell induces the release of electron-dense cytoplasmic granules by the effector cells.	bind
56337	7	6669	6	10	NULL	0	NULL	statement 4			is an alternative to					statement 5					NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_6_1805_s_23	10362805	15  In this pathway, the recognition and tight binding of a susceptible target cell by a CTL or NK cell induces the release of electron-dense cytoplasmic granules by the effector cells.	bind
56338	8	6669	6	10	NULL	0	NULL	statement 6			induces					statement 3					NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_6_1805_s_23	10362805	15  In this pathway, the recognition and tight binding of a susceptible target cell by a CTL or NK cell induces the release of electron-dense cytoplasmic granules by the effector cells.	bind
56339	9	6669	6	10	NULL	0	NULL	statement 7			induces					statement 3					NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_6_1805_s_23	10362805	15  In this pathway, the recognition and tight binding of a susceptible target cell by a CTL or NK cell induces the release of electron-dense cytoplasmic granules by the effector cells.	bind
21710	1	6670	5	13	NULL	NULL	NULL	MS1 cells	Cell		bind					VEGF 165	GP	radio-iodinated			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_4_1469_s_84	10751370	15  MS1 and SVR cells were found to bind radio-iodinated VEGF 165, yielding a band consistent with the combined molecular weight of VEGF and VEGFR-2 after cross-linking (data not shown).	bind
21711	2	6670	5	13	NULL	NULL	NULL	SVR cells	Cell		bind					VEGF 165	GP	radio-iodinated			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_4_1469_s_84	10751370	15  MS1 and SVR cells were found to bind radio-iodinated VEGF 165, yielding a band consistent with the combined molecular weight of VEGF and VEGFR-2 after cross-linking (data not shown).	bind
18793	1	6670	6	NULL	NULL	0	NULL	MS1	NULL		bind	NULL				VEGF 165	NULL	radio-iodinated			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_4_1469_s_84	10751370	15  MS1 and SVR cells were found to bind radio-iodinated VEGF 165, yielding a band consistent with the combined molecular weight of VEGF and VEGFR-2 after cross-linking (data not shown).	bind
18794	2	6670	6	NULL	NULL	0	NULL	SVR cells	NULL		bind	NULL				VEGF 165	NULL	radio-iodinated			NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_4_1469_s_84	10751370	15  MS1 and SVR cells were found to bind radio-iodinated VEGF 165, yielding a band consistent with the combined molecular weight of VEGF and VEGFR-2 after cross-linking (data not shown).	bind
21713	1	6671	5	13	NULL	NULL	NULL	tuberin	GP		bind			59-amino-acid motif in C-terminus		rabaptin-5	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_10_1069_s_34	10827137	15  Other studies identified a 59-amino-acid motif located at the C-terminus of tuberin that binds to rabaptin-5.	bind
18795	1	6671	6	NULL	NULL	0	NULL	tuberin	NULL		bind	NULL		59-amino-acid motif at C-terminus		rabaptin-5	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_86_10_1069_s_34	10827137	15  Other studies identified a 59-amino-acid motif located at the C-terminus of tuberin that binds to rabaptin-5.	bind
21716	1	6672	5	13	NULL	NULL	NULL	PrPL	GP		is					ligand of PrPC	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_5_1447_s_111	11073804	15  They hypothesized two putative molecules; one is a ligand of PrPC (PrPL) eliciting a signal necessary for the survival of neurons, and the other is protein pi that binds to PrPL with lower affinity but also capable of generating the survival signal.	bind
21717	2	6672	5	13	NULL	NULL	NULL	PrPL	GP		signals for					neuronal survival	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_5_1447_s_111	11073804	15  They hypothesized two putative molecules; one is a ligand of PrPC (PrPL) eliciting a signal necessary for the survival of neurons, and the other is protein pi that binds to PrPL with lower affinity but also capable of generating the survival signal.	bind
21718	3	6672	5	13	NULL	NULL	NULL	protein pi	GP		bind		low affinity			PrPL	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_5_1447_s_111	11073804	15  They hypothesized two putative molecules; one is a ligand of PrPC (PrPL) eliciting a signal necessary for the survival of neurons, and the other is protein pi that binds to PrPL with lower affinity but also capable of generating the survival signal.	bind
21720	4	6672	5	13	NULL	NULL	NULL	protein pi	GP		generates					survival signal	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_5_1447_s_111	11073804	15  They hypothesized two putative molecules; one is a ligand of PrPC (PrPL) eliciting a signal necessary for the survival of neurons, and the other is protein pi that binds to PrPL with lower affinity but also capable of generating the survival signal.	bind
18796	1	6672	6	NULL	NULL	0	NULL	protein pi	NULL		bind	NULL	low affinity			PrPL	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_5_1447_s_111	11073804	15  They hypothesized two putative molecules; one is a ligand of PrPC (PrPL) eliciting a signal necessary for the survival of neurons, and the other is protein pi that binds to PrPL with lower affinity but also capable of generating the survival signal.	bind
18797	2	6672	6	NULL	NULL	0	NULL	PrPL	NULL		is	NULL				ligand of PrPC	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_5_1447_s_111	11073804	15  They hypothesized two putative molecules; one is a ligand of PrPC (PrPL) eliciting a signal necessary for the survival of neurons, and the other is protein pi that binds to PrPL with lower affinity but also capable of generating the survival signal.	bind
18798	3	6672	6	NULL	NULL	0	NULL	PrPL	NULL		plays a role in	NULL				neuron survival	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_5_1447_s_111	11073804	15  They hypothesized two putative molecules; one is a ligand of PrPC (PrPL) eliciting a signal necessary for the survival of neurons, and the other is protein pi that binds to PrPL with lower affinity but also capable of generating the survival signal.	bind
18799	4	6672	6	10	NULL	0	NULL	protein pi			play a role in					 survival signal					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_5_1447_s_111	11073804	15  They hypothesized two putative molecules; one is a ligand of PrPC (PrPL) eliciting a signal necessary for the survival of neurons, and the other is protein pi that binds to PrPL with lower affinity but also capable of generating the survival signal.	bind
21722	1	6673	5	13	NULL	NULL	NULL	SV40 LT antigen	GP		bind					p53	GP	wild-type			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_973_s_102	10764661	15  Those studies also established that SV40 LT antigen binds to wild-type p53 and extends its half-life.	bind
21723	2	6673	5	13	NULL	NULL	NULL	statement 1	Process		extends					p53	GP	half life of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_973_s_102	10764661	15  Those studies also established that SV40 LT antigen binds to wild-type p53 and extends its half-life.	bind
18800	1	6673	6	NULL	NULL	0	NULL	SV40 LT antigen	NULL		bind	NULL				p53	NULL	wild type			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_973_s_102	10764661	15  Those studies also established that SV40 LT antigen binds to wild-type p53 and extends its half-life.	bind
31149	2	6673	6	10	NULL	0	NULL	statement 1			extends					p53 		half life of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_973_s_102	10764661	15  Those studies also established that SV40 LT antigen binds to wild-type p53 and extends its half-life.	bind
21724	1	6674	5	13	NULL	NULL	NULL	SV40 LT antigen	GP		bind					p53	GP	wild-type			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_3_636_s_105	10712385	15  Those studies have also established that SV40 LT antigen binds to wild-type p53 and extends its half-life.	bind
21725	2	6674	5	13	NULL	NULL	NULL	SV40 LT antigen	GP		extends					p53	GP	half life of wild-type			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_3_636_s_105	10712385	15  Those studies have also established that SV40 LT antigen binds to wild-type p53 and extends its half-life.	bind
21726	1	6675	5	13	NULL	NULL	NULL	annexin V	GP		bind					 phospholipid	Chemical	anionic			NULL	on platelets	NULL	NULL	NULL	NULL	gw60_circulation_96_7_2339_s_32	9337209	15  We have shown previously that annexin V binds to anionic phospholipid on platelets and blocks the binding of factors Xa and Va to platelets.	bind
21727	2	6675	5	13	NULL	NULL	NULL	factor Xa	GP		bind					platelets	Cell				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_7_2339_s_32	9337209	15  We have shown previously that annexin V binds to anionic phospholipid on platelets and blocks the binding of factors Xa and Va to platelets.	bind
21728	3	6675	5	13	NULL	NULL	NULL	factor Va	GP		bind					platelets	Cell				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_7_2339_s_32	9337209	15  We have shown previously that annexin V binds to anionic phospholipid on platelets and blocks the binding of factors Xa and Va to platelets.	bind
21729	4	6675	5	13	NULL	NULL	NULL	statement 1	Process		blocks					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_7_2339_s_32	9337209	15  We have shown previously that annexin V binds to anionic phospholipid on platelets and blocks the binding of factors Xa and Va to platelets.	bind
21730	5	6675	5	13	NULL	NULL	NULL	statement 1	Process		blocks					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_7_2339_s_32	9337209	15  We have shown previously that annexin V binds to anionic phospholipid on platelets and blocks the binding of factors Xa and Va to platelets.	bind
18801	1	6675	6	NULL	NULL	0	NULL	annexin V	NULL		bind	NULL				phospholipids	NULL	anionic			NULL	platelets	0	NULL	NULL	NULL	gw60_circulation_96_7_2339_s_32	9337209	15  We have shown previously that annexin V binds to anionic phospholipid on platelets and blocks the binding of factors Xa and Va to platelets.	bind
18802	2	6675	6	NULL	NULL	0	NULL	factor Xa	NULL		bind	NULL				platelets	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_96_7_2339_s_32	9337209	15  We have shown previously that annexin V binds to anionic phospholipid on platelets and blocks the binding of factors Xa and Va to platelets.	bind
18803	3	6675	6	NULL	NULL	0	NULL	factor Va	NULL		bind	NULL				platelets	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_96_7_2339_s_32	9337209	15  We have shown previously that annexin V binds to anionic phospholipid on platelets and blocks the binding of factors Xa and Va to platelets.	bind
18804	4	6675	6	NULL	NULL	0	NULL	statement 1	NULL		blocks	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_96_7_2339_s_32	9337209	15  We have shown previously that annexin V binds to anionic phospholipid on platelets and blocks the binding of factors Xa and Va to platelets.	bind
18805	5	6675	6	NULL	NULL	0	NULL	statement 1	NULL		blocks	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_96_7_2339_s_32	9337209	15  We have shown previously that annexin V binds to anionic phospholipid on platelets and blocks the binding of factors Xa and Va to platelets.	bind
24797	1	6676	5	13	NULL	NULL	NULL	F1F0-ATPase	GP	natural inhibitor of	bind					F1F0-ATPase	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_29	15345651	15 - 19     In fact, many cells contain a natural inhibitor of the F1F0-ATPase, which binds the F1F0-ATPase during ischemia to inhibit breakdown of glycolytic ATP. 20 There are also data showing that ischemia and anoxia lead to a preferential decrease in cytosolic versus mitochondrial ATP, 21,22  suggesting that cells may regulate mitochondrial ADP/ATP exchange during ischemia.	bind
24798	2	6676	5	13	NULL	NULL	NULL	statement 1	Process		inhibit					glycolytic ATP	Chemical	breakdown of 			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_29	15345651	15 - 19     In fact, many cells contain a natural inhibitor of the F1F0-ATPase, which binds the F1F0-ATPase during ischemia to inhibit breakdown of glycolytic ATP. 20 There are also data showing that ischemia and anoxia lead to a preferential decrease in cytosolic versus mitochondrial ATP, 21,22  suggesting that cells may regulate mitochondrial ADP/ATP exchange during ischemia.	bind
24799	3	6676	5	13	NULL	NULL	NULL	ischemia	MedicalFinding		leads to					ATP	Chemical	preferential decrease in cytosolic			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_29	15345651	15 - 19     In fact, many cells contain a natural inhibitor of the F1F0-ATPase, which binds the F1F0-ATPase during ischemia to inhibit breakdown of glycolytic ATP. 20 There are also data showing that ischemia and anoxia lead to a preferential decrease in cytosolic versus mitochondrial ATP, 21,22  suggesting that cells may regulate mitochondrial ADP/ATP exchange during ischemia.	bind
24800	4	6676	5	13	NULL	NULL	NULL	ischemia	MedicalFinding		leads to					ATP	Chemical	preferential decrease in mitochondrial			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_29	15345651	15 - 19     In fact, many cells contain a natural inhibitor of the F1F0-ATPase, which binds the F1F0-ATPase during ischemia to inhibit breakdown of glycolytic ATP. 20 There are also data showing that ischemia and anoxia lead to a preferential decrease in cytosolic versus mitochondrial ATP, 21,22  suggesting that cells may regulate mitochondrial ADP/ATP exchange during ischemia.	bind
24801	5	6676	5	13	NULL	NULL	NULL	anoxia	MedicalFinding		leads to					ATP	Chemical	preferential decrease in cytosolic			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_29	15345651	15 - 19     In fact, many cells contain a natural inhibitor of the F1F0-ATPase, which binds the F1F0-ATPase during ischemia to inhibit breakdown of glycolytic ATP. 20 There are also data showing that ischemia and anoxia lead to a preferential decrease in cytosolic versus mitochondrial ATP, 21,22  suggesting that cells may regulate mitochondrial ADP/ATP exchange during ischemia.	bind
24802	6	6676	5	13	NULL	NULL	NULL	anoxia	MedicalFinding		leads to					ATP	Chemical	preferential decrease in mitochondrial			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_29	15345651	15 - 19     In fact, many cells contain a natural inhibitor of the F1F0-ATPase, which binds the F1F0-ATPase during ischemia to inhibit breakdown of glycolytic ATP. 20 There are also data showing that ischemia and anoxia lead to a preferential decrease in cytosolic versus mitochondrial ATP, 21,22  suggesting that cells may regulate mitochondrial ADP/ATP exchange during ischemia.	bind
24803	7	6676	5	13	NULL	NULL	NULL	cells	Cell		regulates		may			ADP/ATP	Chemical	mitochondrial;;exchange of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_29	15345651	15 - 19     In fact, many cells contain a natural inhibitor of the F1F0-ATPase, which binds the F1F0-ATPase during ischemia to inhibit breakdown of glycolytic ATP. 20 There are also data showing that ischemia and anoxia lead to a preferential decrease in cytosolic versus mitochondrial ATP, 21,22  suggesting that cells may regulate mitochondrial ADP/ATP exchange during ischemia.	bind
24805	8	6676	5	13	NULL	NULL	NULL	statement 3	Process		suggests					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_29	15345651	15 - 19     In fact, many cells contain a natural inhibitor of the F1F0-ATPase, which binds the F1F0-ATPase during ischemia to inhibit breakdown of glycolytic ATP. 20 There are also data showing that ischemia and anoxia lead to a preferential decrease in cytosolic versus mitochondrial ATP, 21,22  suggesting that cells may regulate mitochondrial ADP/ATP exchange during ischemia.	bind
24806	9	6676	5	13	NULL	NULL	NULL	statement 4	Process		suggests					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_29	15345651	15 - 19     In fact, many cells contain a natural inhibitor of the F1F0-ATPase, which binds the F1F0-ATPase during ischemia to inhibit breakdown of glycolytic ATP. 20 There are also data showing that ischemia and anoxia lead to a preferential decrease in cytosolic versus mitochondrial ATP, 21,22  suggesting that cells may regulate mitochondrial ADP/ATP exchange during ischemia.	bind
24807	10	6676	5	13	NULL	NULL	NULL	statement 5	Process		suggests					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_29	15345651	15 - 19     In fact, many cells contain a natural inhibitor of the F1F0-ATPase, which binds the F1F0-ATPase during ischemia to inhibit breakdown of glycolytic ATP. 20 There are also data showing that ischemia and anoxia lead to a preferential decrease in cytosolic versus mitochondrial ATP, 21,22  suggesting that cells may regulate mitochondrial ADP/ATP exchange during ischemia.	bind
24808	11	6676	5	13	NULL	NULL	NULL	statement 6	Process		suggests					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_29	15345651	15 - 19     In fact, many cells contain a natural inhibitor of the F1F0-ATPase, which binds the F1F0-ATPase during ischemia to inhibit breakdown of glycolytic ATP. 20 There are also data showing that ischemia and anoxia lead to a preferential decrease in cytosolic versus mitochondrial ATP, 21,22  suggesting that cells may regulate mitochondrial ADP/ATP exchange during ischemia.	bind
56350	12	6676	5	13	NULL	NULL	NULL	statement 1	Process		occur during					ischemia	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_29	15345651	15 - 19     In fact, many cells contain a natural inhibitor of the F1F0-ATPase, which binds the F1F0-ATPase during ischemia to inhibit breakdown of glycolytic ATP. 20 There are also data showing that ischemia and anoxia lead to a preferential decrease in cytosolic versus mitochondrial ATP, 21,22  suggesting that cells may regulate mitochondrial ADP/ATP exchange during ischemia.	bind
56351	13	6676	5	13	NULL	NULL	NULL	statement 7	Process		occur during					ischemia	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_29	15345651	15 - 19     In fact, many cells contain a natural inhibitor of the F1F0-ATPase, which binds the F1F0-ATPase during ischemia to inhibit breakdown of glycolytic ATP. 20 There are also data showing that ischemia and anoxia lead to a preferential decrease in cytosolic versus mitochondrial ATP, 21,22  suggesting that cells may regulate mitochondrial ADP/ATP exchange during ischemia.	bind
18987	1	6676	6	10	NULL	0	NULL	F1F0-ATPase		natural inhibitor of	bind					F1F0-ATPase					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_29	15345651	15 - 19     In fact, many cells contain a natural inhibitor of the F1F0-ATPase, which binds the F1F0-ATPase during ischemia to inhibit breakdown of glycolytic ATP. 20 There are also data showing that ischemia and anoxia lead to a preferential decrease in cytosolic versus mitochondrial ATP, 21,22  suggesting that cells may regulate mitochondrial ADP/ATP exchange during ischemia.	bind
18988	2	6676	6	NULL	NULL	0	NULL	statement 1	NULL		occurs during	NULL				ischemia	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_29	15345651	15 - 19     In fact, many cells contain a natural inhibitor of the F1F0-ATPase, which binds the F1F0-ATPase during ischemia to inhibit breakdown of glycolytic ATP. 20 There are also data showing that ischemia and anoxia lead to a preferential decrease in cytosolic versus mitochondrial ATP, 21,22  suggesting that cells may regulate mitochondrial ADP/ATP exchange during ischemia.	bind
18991	3	6676	6	NULL	NULL	0	NULL	statement 1	NULL		inhibit	NULL				glycolytic ATP	NULL	breakdown of 			NULL		0	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_29	15345651	15 - 19     In fact, many cells contain a natural inhibitor of the F1F0-ATPase, which binds the F1F0-ATPase during ischemia to inhibit breakdown of glycolytic ATP. 20 There are also data showing that ischemia and anoxia lead to a preferential decrease in cytosolic versus mitochondrial ATP, 21,22  suggesting that cells may regulate mitochondrial ADP/ATP exchange during ischemia.	bind
56340	4	6676	6	10	NULL	0	NULL	 ischemia 			lead to					ATP		preferential decrease in cytosolic			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_29	15345651	15 - 19     In fact, many cells contain a natural inhibitor of the F1F0-ATPase, which binds the F1F0-ATPase during ischemia to inhibit breakdown of glycolytic ATP. 20 There are also data showing that ischemia and anoxia lead to a preferential decrease in cytosolic versus mitochondrial ATP, 21,22  suggesting that cells may regulate mitochondrial ADP/ATP exchange during ischemia.	bind
56341	5	6676	6	10	NULL	0	NULL	ischemia			lead to					ATP		preferential decrease in mitochondrial			NULL		0	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_29	15345651	15 - 19     In fact, many cells contain a natural inhibitor of the F1F0-ATPase, which binds the F1F0-ATPase during ischemia to inhibit breakdown of glycolytic ATP. 20 There are also data showing that ischemia and anoxia lead to a preferential decrease in cytosolic versus mitochondrial ATP, 21,22  suggesting that cells may regulate mitochondrial ADP/ATP exchange during ischemia.	bind
56342	6	6676	6	10	NULL	0	NULL	anoxia 			lead to					ATP		preferential decrease in cytosolic			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_29	15345651	15 - 19     In fact, many cells contain a natural inhibitor of the F1F0-ATPase, which binds the F1F0-ATPase during ischemia to inhibit breakdown of glycolytic ATP. 20 There are also data showing that ischemia and anoxia lead to a preferential decrease in cytosolic versus mitochondrial ATP, 21,22  suggesting that cells may regulate mitochondrial ADP/ATP exchange during ischemia.	bind
56343	7	6676	6	10	NULL	0	NULL	anoxia 			lead to					ATP		preferential decrease in mitochondrial			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_29	15345651	15 - 19     In fact, many cells contain a natural inhibitor of the F1F0-ATPase, which binds the F1F0-ATPase during ischemia to inhibit breakdown of glycolytic ATP. 20 There are also data showing that ischemia and anoxia lead to a preferential decrease in cytosolic versus mitochondrial ATP, 21,22  suggesting that cells may regulate mitochondrial ADP/ATP exchange during ischemia.	bind
56344	8	6676	6	10	NULL	0	NULL	cells			regulate		may			ADP/ATP		mitochondrial;;exchange of			NULL		0	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_29	15345651	15 - 19     In fact, many cells contain a natural inhibitor of the F1F0-ATPase, which binds the F1F0-ATPase during ischemia to inhibit breakdown of glycolytic ATP. 20 There are also data showing that ischemia and anoxia lead to a preferential decrease in cytosolic versus mitochondrial ATP, 21,22  suggesting that cells may regulate mitochondrial ADP/ATP exchange during ischemia.	bind
56345	9	6676	6	10	NULL	0	NULL	statement 8			occur during					ischemia					NULL		0	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_29	15345651	15 - 19     In fact, many cells contain a natural inhibitor of the F1F0-ATPase, which binds the F1F0-ATPase during ischemia to inhibit breakdown of glycolytic ATP. 20 There are also data showing that ischemia and anoxia lead to a preferential decrease in cytosolic versus mitochondrial ATP, 21,22  suggesting that cells may regulate mitochondrial ADP/ATP exchange during ischemia.	bind
56346	10	6676	6	10	NULL	0	NULL	statement 4			suggest					statement 8					NULL		0	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_29	15345651	15 - 19     In fact, many cells contain a natural inhibitor of the F1F0-ATPase, which binds the F1F0-ATPase during ischemia to inhibit breakdown of glycolytic ATP. 20 There are also data showing that ischemia and anoxia lead to a preferential decrease in cytosolic versus mitochondrial ATP, 21,22  suggesting that cells may regulate mitochondrial ADP/ATP exchange during ischemia.	bind
56347	11	6676	6	10	NULL	0	NULL	statement 5			suggest					statement 8					NULL		0	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_29	15345651	15 - 19     In fact, many cells contain a natural inhibitor of the F1F0-ATPase, which binds the F1F0-ATPase during ischemia to inhibit breakdown of glycolytic ATP. 20 There are also data showing that ischemia and anoxia lead to a preferential decrease in cytosolic versus mitochondrial ATP, 21,22  suggesting that cells may regulate mitochondrial ADP/ATP exchange during ischemia.	bind
56348	12	6676	6	10	NULL	0	NULL	statement 6			suggest					statement 8					NULL		0	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_29	15345651	15 - 19     In fact, many cells contain a natural inhibitor of the F1F0-ATPase, which binds the F1F0-ATPase during ischemia to inhibit breakdown of glycolytic ATP. 20 There are also data showing that ischemia and anoxia lead to a preferential decrease in cytosolic versus mitochondrial ATP, 21,22  suggesting that cells may regulate mitochondrial ADP/ATP exchange during ischemia.	bind
56349	13	6676	6	10	NULL	0	NULL	statement 7			suggest					statement 8					NULL		0	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_29	15345651	15 - 19     In fact, many cells contain a natural inhibitor of the F1F0-ATPase, which binds the F1F0-ATPase during ischemia to inhibit breakdown of glycolytic ATP. 20 There are also data showing that ischemia and anoxia lead to a preferential decrease in cytosolic versus mitochondrial ATP, 21,22  suggesting that cells may regulate mitochondrial ADP/ATP exchange during ischemia.	bind
21731	1	6677	5	13	NULL	NULL	NULL	Endoglin	GP		does not bind					TGF-beta1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_12_2546_s_38	11116051	15 16  Endoglin alone does not bind TGF-beta1 or -beta3 but requires the presence of TbetaR-II.	bind
21732	2	6677	5	13	NULL	NULL	NULL	Endoglin	GP		does not bind					TGF-beta3	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_12_2546_s_38	11116051	15 16  Endoglin alone does not bind TGF-beta1 or -beta3 but requires the presence of TbetaR-II.	bind
21733	3	6677	5	13	NULL	NULL	NULL	Endoglin	GP		bind					TGF-beta1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_12_2546_s_38	11116051	15 16  Endoglin alone does not bind TGF-beta1 or -beta3 but requires the presence of TbetaR-II.	bind
21734	4	6677	5	13	NULL	NULL	NULL	statement 3	Process		in the presence of					TbetaR-II	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_12_2546_s_38	11116051	15 16  Endoglin alone does not bind TGF-beta1 or -beta3 but requires the presence of TbetaR-II.	bind
21735	5	6677	5	13	NULL	NULL	NULL	Endoglin	GP		bind					TGF-beta3	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_12_2546_s_38	11116051	15 16  Endoglin alone does not bind TGF-beta1 or -beta3 but requires the presence of TbetaR-II.	bind
21736	6	6677	5	13	NULL	NULL	NULL	statement 5	Process		in the presence of					TbetaR-II	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_12_2546_s_38	11116051	15 16  Endoglin alone does not bind TGF-beta1 or -beta3 but requires the presence of TbetaR-II.	bind
18806	1	6677	6	NULL	NULL	0	NULL	Endoglin	NULL		bind	NULL				TGF-beta1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_12_2546_s_38	11116051	15 16  Endoglin alone does not bind TGF-beta1 or -beta3 but requires the presence of TbetaR-II.	bind
18807	2	6677	6	NULL	NULL	0	NULL	Endoglin	NULL		bind	NULL				TGF-beta3	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_12_2546_s_38	11116051	15 16  Endoglin alone does not bind TGF-beta1 or -beta3 but requires the presence of TbetaR-II.	bind
18808	3	6677	6	NULL	NULL	0	NULL	statement 1	NULL		occurs in presence of	NULL	only			TbetaR-II	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_12_2546_s_38	11116051	15 16  Endoglin alone does not bind TGF-beta1 or -beta3 but requires the presence of TbetaR-II.	bind
18809	4	6677	6	NULL	NULL	0	NULL	statement 2	NULL		occurs in presence of	NULL	only			TbetaR-II	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_12_2546_s_38	11116051	15 16  Endoglin alone does not bind TGF-beta1 or -beta3 but requires the presence of TbetaR-II.	bind
21737	1	6678	5	13	NULL	NULL	NULL	Heparin	Chemical		bind		avidly			smooth muscle cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_6_1143_s_209	7586227	15 17  Heparin avidly binds to smooth muscle cells and extracellular structures.	bind
21738	2	6678	5	13	NULL	NULL	NULL	Heparin	Chemical		bind		avidly			extracellular structures	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_6_1143_s_209	7586227	15 17  Heparin avidly binds to smooth muscle cells and extracellular structures.	bind
18810	1	6678	6	NULL	NULL	0	NULL	heparin	NULL		bind	NULL	avidly			smooth muscle cells	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_77_6_1143_s_209	7586227	15 17  Heparin avidly binds to smooth muscle cells and extracellular structures.	bind
18811	2	6678	6	NULL	NULL	0	NULL	heparin	NULL		bind	NULL	avidly			extracellular structures	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_77_6_1143_s_209	7586227	15 17  Heparin avidly binds to smooth muscle cells and extracellular structures.	bind
21740	1	6681	5	13	NULL	NULL	NULL	SREBP-2	GP		bind		exclusively			squalene synthase	NucleicAcid	human		SRE 5''-TCCACCCCAC-3''	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2358_s_156	15486308	15 Conversely, it has also been suggested that differences in the first 2 5' nucleotides of the LDL-receptor SRE-1 could explain the exclusive binding of SREBP-2 to the human squalene synthase SRE (8/10) 5''-TCCACCCCAC-3''.	bind
21743	2	6681	5	13	NULL	NULL	NULL	LDL-receptor	GP	differences of	explains				SRE-1 nucleotides	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2358_s_156	15486308	15 Conversely, it has also been suggested that differences in the first 2 5' nucleotides of the LDL-receptor SRE-1 could explain the exclusive binding of SREBP-2 to the human squalene synthase SRE (8/10) 5''-TCCACCCCAC-3''.	bind
18812	1	6681	6	NULL	NULL	0	NULL	SREBP-2	NULL		bind	NULL	exclusively			squalene synthase	NULL	human		SRE (8/10)-TCCACCCCAC	NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2358_s_156	15486308	15 Conversely, it has also been suggested that differences in the first 2 5' nucleotides of the LDL-receptor SRE-1 could explain the exclusive binding of SREBP-2 to the human squalene synthase SRE (8/10) 5''-TCCACCCCAC-3''.	bind
30470	2	6681	6	NULL	NULL	0	NULL	LDL receptor	NULL	difference of	explains	NULL			SRE-1 nucleotides	statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2358_s_156	15486308	15 Conversely, it has also been suggested that differences in the first 2 5' nucleotides of the LDL-receptor SRE-1 could explain the exclusive binding of SREBP-2 to the human squalene synthase SRE (8/10) 5''-TCCACCCCAC-3''.	bind
21744	1	6682	5	13	NULL	NULL	NULL	DDAH1	GP		bind					NF1	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1419_s_33	16794231	15 DDAH1 binding to NF1 promoted the phosphorylation of NF1 by PKA at specific residues within the cysteine/serine rich domain.	bind
21745	2	6682	5	13	NULL	NULL	NULL	PKA	GP		phosphorylates					NF1	GP		specific residues within the  cysteine/serine rich domain		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1419_s_33	16794231	15 DDAH1 binding to NF1 promoted the phosphorylation of NF1 by PKA at specific residues within the cysteine/serine rich domain.	bind
21746	3	6682	5	13	NULL	NULL	NULL	statement 1	Process		promote					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1419_s_33	16794231	15 DDAH1 binding to NF1 promoted the phosphorylation of NF1 by PKA at specific residues within the cysteine/serine rich domain.	bind
18813	1	6682	6	NULL	NULL	0	NULL	DDAH1	NULL		bind	NULL				NF1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1419_s_33	16794231	15 DDAH1 binding to NF1 promoted the phosphorylation of NF1 by PKA at specific residues within the cysteine/serine rich domain.	bind
18814	2	6682	6	NULL	NULL	0	NULL	PKA	NULL		phosphorylates	NULL				NF1	NULL		specific residues within the cysteine/serine rich domain		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1419_s_33	16794231	15 DDAH1 binding to NF1 promoted the phosphorylation of NF1 by PKA at specific residues within the cysteine/serine rich domain.	bind
18815	3	6682	6	NULL	NULL	0	NULL	statement 1	NULL		promotes	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1419_s_33	16794231	15 DDAH1 binding to NF1 promoted the phosphorylation of NF1 by PKA at specific residues within the cysteine/serine rich domain.	bind
21748	1	6683	5	13	NULL	NULL	NULL	fibrinogen	GP		bind					GPIIb-IIIa	GP	activated			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_1_252_s_171	15514209	15 Despite a larger number of heterozygotes and homozygotes for the minor haplotype in our study, we did not detect any effect of this variant on fibrinogen binding to activated GPIIb-IIIa.	bind
18816	1	6683	6	NULL	NULL	0	NULL	fibrinogen	NULL		bind	NULL				GPIIb-IIIa	NULL	activated			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_1_252_s_171	15514209	15 Despite a larger number of heterozygotes and homozygotes for the minor haplotype in our study, we did not detect any effect of this variant on fibrinogen binding to activated GPIIb-IIIa.	bind
21749	1	6684	5	13	NULL	NULL	NULL	CKIs	GP		is					cyclin-dependent kinase inhibitors	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_511_s_33	14726409	15 Furthermore, cell cycle progression is regulated by the expression of cyclin-dependent kinase inhibitors (CKIs) such as p27kip1 and p21waf, which bind to CDKs and prevent their activation 14,15	bind
21751	2	6684	5	13	NULL	NULL	NULL	p27kip1	GP		is a type of					CKIs	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_511_s_33	14726409	15 Furthermore, cell cycle progression is regulated by the expression of cyclin-dependent kinase inhibitors (CKIs) such as p27kip1 and p21waf, which bind to CDKs and prevent their activation 14,15	bind
21752	3	6684	5	13	NULL	NULL	NULL	p21waf	GP		is a type of					CKIs	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_511_s_33	14726409	15 Furthermore, cell cycle progression is regulated by the expression of cyclin-dependent kinase inhibitors (CKIs) such as p27kip1 and p21waf, which bind to CDKs and prevent their activation 14,15	bind
21754	4	6684	5	13	NULL	NULL	NULL	p27kip1	GP		bind					CDKs	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_511_s_33	14726409	15 Furthermore, cell cycle progression is regulated by the expression of cyclin-dependent kinase inhibitors (CKIs) such as p27kip1 and p21waf, which bind to CDKs and prevent their activation 14,15	bind
21755	5	6684	5	13	NULL	NULL	NULL	statement 4	Process		prevents					CDKs	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_511_s_33	14726409	15 Furthermore, cell cycle progression is regulated by the expression of cyclin-dependent kinase inhibitors (CKIs) such as p27kip1 and p21waf, which bind to CDKs and prevent their activation 14,15	bind
21756	6	6684	5	13	NULL	NULL	NULL	p21waf	GP		bind					CDKs	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_511_s_33	14726409	15 Furthermore, cell cycle progression is regulated by the expression of cyclin-dependent kinase inhibitors (CKIs) such as p27kip1 and p21waf, which bind to CDKs and prevent their activation 14,15	bind
21758	7	6684	5	13	NULL	NULL	NULL	statement 6	Process		prevents					CDKs	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_511_s_33	14726409	15 Furthermore, cell cycle progression is regulated by the expression of cyclin-dependent kinase inhibitors (CKIs) such as p27kip1 and p21waf, which bind to CDKs and prevent their activation 14,15	bind
21759	8	6684	5	13	NULL	NULL	NULL	CKIs	GP	expression of	regulates					cell cycle 	Process	progression of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_511_s_33	14726409	15 Furthermore, cell cycle progression is regulated by the expression of cyclin-dependent kinase inhibitors (CKIs) such as p27kip1 and p21waf, which bind to CDKs and prevent their activation 14,15	bind
18817	1	6684	6	NULL	NULL	0	NULL	p27kip1	NULL		bind	NULL				CDK	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_511_s_33	14726409	15 Furthermore, cell cycle progression is regulated by the expression of cyclin-dependent kinase inhibitors (CKIs) such as p27kip1 and p21waf, which bind to CDKs and prevent their activation 14,15	bind
18818	2	6684	6	NULL	NULL	0	NULL	p21waf	NULL		bind	NULL				CDK	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_511_s_33	14726409	15 Furthermore, cell cycle progression is regulated by the expression of cyclin-dependent kinase inhibitors (CKIs) such as p27kip1 and p21waf, which bind to CDKs and prevent their activation 14,15	bind
18819	3	6684	6	NULL	NULL	0	NULL	p27kip1	NULL		is a type of	NULL				CKI	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_511_s_33	14726409	15 Furthermore, cell cycle progression is regulated by the expression of cyclin-dependent kinase inhibitors (CKIs) such as p27kip1 and p21waf, which bind to CDKs and prevent their activation 14,15	bind
18820	4	6684	6	NULL	NULL	0	NULL	CKI	NULL		is	NULL				cyclin dependent kinase inhibitors	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_511_s_33	14726409	15 Furthermore, cell cycle progression is regulated by the expression of cyclin-dependent kinase inhibitors (CKIs) such as p27kip1 and p21waf, which bind to CDKs and prevent their activation 14,15	bind
18821	5	6684	6	NULL	NULL	0	NULL	p21waf1	NULL		is a type of	NULL				CKI	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_511_s_33	14726409	15 Furthermore, cell cycle progression is regulated by the expression of cyclin-dependent kinase inhibitors (CKIs) such as p27kip1 and p21waf, which bind to CDKs and prevent their activation 14,15	bind
18822	6	6684	6	NULL	NULL	0	NULL	p27kip1	NULL		regulates	NULL				cell cycle 	NULL	progression of 			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_511_s_33	14726409	15 Furthermore, cell cycle progression is regulated by the expression of cyclin-dependent kinase inhibitors (CKIs) such as p27kip1 and p21waf, which bind to CDKs and prevent their activation 14,15	bind
18823	7	6684	6	NULL	NULL	0	NULL	p21waf1	NULL		regulates	NULL				cell cycle 	NULL	progression of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_511_s_33	14726409	15 Furthermore, cell cycle progression is regulated by the expression of cyclin-dependent kinase inhibitors (CKIs) such as p27kip1 and p21waf, which bind to CDKs and prevent their activation 14,15	bind
30471	8	6684	6	NULL	NULL	0	NULL	statement 1	NULL		prevents	NULL				CDK	NULL	activation of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_511_s_33	14726409	15 Furthermore, cell cycle progression is regulated by the expression of cyclin-dependent kinase inhibitors (CKIs) such as p27kip1 and p21waf, which bind to CDKs and prevent their activation 14,15	bind
30472	9	6684	6	NULL	NULL	0	NULL	statement 2	NULL		prevents	NULL				CDK	NULL	activation of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_511_s_33	14726409	15 Furthermore, cell cycle progression is regulated by the expression of cyclin-dependent kinase inhibitors (CKIs) such as p27kip1 and p21waf, which bind to CDKs and prevent their activation 14,15	bind
21761	1	6685	5	13	NULL	NULL	NULL	Grp78	GP		bind		transiently			proteins	GP	newly synthesized			NULL	ER	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_3_571_s_31	15618547	15 Grp78 binds transiently to newly synthesized proteins in the ER and more permanently to misfolded unglycosylated proteins whose transport from the ER is blocked.	bind
21764	2	6685	5	13	NULL	NULL	NULL	Grp78	GP		bind		permanently			proteins	GP	misfolded;;unglycosylated			NULL	ER	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_3_571_s_31	15618547	15 Grp78 binds transiently to newly synthesized proteins in the ER and more permanently to misfolded unglycosylated proteins whose transport from the ER is blocked.	bind
18824	1	6685	6	10	NULL	0	NULL	Grp78	NULL		bind	NULL	transiently			 proteins	NULL	newly synthesized			NULL	ER	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_3_571_s_31	15618547	15 Grp78 binds transiently to newly synthesized proteins in the ER and more permanently to misfolded unglycosylated proteins whose transport from the ER is blocked.	bind
18825	2	6685	6	10	NULL	0	NULL	Grp78			bind		permanently			protein		misfolded;;unglycosylated			NULL	ER	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_3_571_s_31	15618547	15 Grp78 binds transiently to newly synthesized proteins in the ER and more permanently to misfolded unglycosylated proteins whose transport from the ER is blocked.	bind
21765	1	6686	5	13	NULL	NULL	NULL	HSPGs	GP		bind					bFGF	GP				NULL	 pericellular matrix	NULL	NULL	NULL	NULL	gw70_circulationres_94_3_340_s_152	14670838	15 Heparin inhibits FGF signaling by competing with HSPGs for binding bFGF. 15,28  Our data suggest that bFGF is released from the cells after stimulation with thrombin and FXa and binds to HSPGs in the pericellular matrix ( Figures 4A and 5   ).	bind
21766	2	6686	5	13	NULL	NULL	NULL	Heparin	Chemical		bind					bFGF	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_340_s_152	14670838	15 Heparin inhibits FGF signaling by competing with HSPGs for binding bFGF. 15,28  Our data suggest that bFGF is released from the cells after stimulation with thrombin and FXa and binds to HSPGs in the pericellular matrix ( Figures 4A and 5   ).	bind
21767	3	6686	5	13	NULL	NULL	NULL	statement 2	Process		competes with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_340_s_152	14670838	15 Heparin inhibits FGF signaling by competing with HSPGs for binding bFGF. 15,28  Our data suggest that bFGF is released from the cells after stimulation with thrombin and FXa and binds to HSPGs in the pericellular matrix ( Figures 4A and 5   ).	bind
21768	4	6686	5	13	NULL	NULL	NULL	Heparin	Chemical		inhibit					FGF	Process	signalling of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_340_s_152	14670838	15 Heparin inhibits FGF signaling by competing with HSPGs for binding bFGF. 15,28  Our data suggest that bFGF is released from the cells after stimulation with thrombin and FXa and binds to HSPGs in the pericellular matrix ( Figures 4A and 5   ).	bind
21769	5	6686	5	13	NULL	NULL	NULL	statement 3	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_340_s_152	14670838	15 Heparin inhibits FGF signaling by competing with HSPGs for binding bFGF. 15,28  Our data suggest that bFGF is released from the cells after stimulation with thrombin and FXa and binds to HSPGs in the pericellular matrix ( Figures 4A and 5   ).	bind
21770	6	6686	5	13	NULL	NULL	NULL	bFGF	GP		released from					cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_340_s_152	14670838	15 Heparin inhibits FGF signaling by competing with HSPGs for binding bFGF. 15,28  Our data suggest that bFGF is released from the cells after stimulation with thrombin and FXa and binds to HSPGs in the pericellular matrix ( Figures 4A and 5   ).	bind
21772	7	6686	5	13	NULL	NULL	NULL	statement 6	Process		occurs after stimulation with					thrombin	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_340_s_152	14670838	15 Heparin inhibits FGF signaling by competing with HSPGs for binding bFGF. 15,28  Our data suggest that bFGF is released from the cells after stimulation with thrombin and FXa and binds to HSPGs in the pericellular matrix ( Figures 4A and 5   ).	bind
21782	9	6686	5	13	NULL	NULL	NULL	statement 7	Process		occurs along with					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_340_s_152	14670838	15 Heparin inhibits FGF signaling by competing with HSPGs for binding bFGF. 15,28  Our data suggest that bFGF is released from the cells after stimulation with thrombin and FXa and binds to HSPGs in the pericellular matrix ( Figures 4A and 5   ).	bind
44669	8	6686	5	13	NULL	NULL	NULL	statement 6	Process		occurs after stimulation with					FXa	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_340_s_152	14670838	15 Heparin inhibits FGF signaling by competing with HSPGs for binding bFGF. 15,28  Our data suggest that bFGF is released from the cells after stimulation with thrombin and FXa and binds to HSPGs in the pericellular matrix ( Figures 4A and 5   ).	bind
56353	10	6686	5	13	NULL	NULL	NULL	statement 1	Process		occurs after					statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_340_s_152	14670838	15 Heparin inhibits FGF signaling by competing with HSPGs for binding bFGF. 15,28  Our data suggest that bFGF is released from the cells after stimulation with thrombin and FXa and binds to HSPGs in the pericellular matrix ( Figures 4A and 5   ).	bind
18826	1	6686	6	NULL	NULL	0	NULL	HSPG	NULL		bind	NULL				bFGF	NULL				NULL	pericellular matrix	NULL	NULL	NULL	NULL	gw70_circulationres_94_3_340_s_152	14670838	15 Heparin inhibits FGF signaling by competing with HSPGs for binding bFGF. 15,28  Our data suggest that bFGF is released from the cells after stimulation with thrombin and FXa and binds to HSPGs in the pericellular matrix ( Figures 4A and 5   ).	bind
18827	2	6686	6	NULL	NULL	0	NULL	heparin	NULL		bind	NULL				bFGF	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_3_340_s_152	14670838	15 Heparin inhibits FGF signaling by competing with HSPGs for binding bFGF. 15,28  Our data suggest that bFGF is released from the cells after stimulation with thrombin and FXa and binds to HSPGs in the pericellular matrix ( Figures 4A and 5   ).	bind
18828	3	6686	6	NULL	NULL	0	NULL	statement 1	NULL		competes	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_3_340_s_152	14670838	15 Heparin inhibits FGF signaling by competing with HSPGs for binding bFGF. 15,28  Our data suggest that bFGF is released from the cells after stimulation with thrombin and FXa and binds to HSPGs in the pericellular matrix ( Figures 4A and 5   ).	bind
18861	4	6686	6	10	NULL	0	NULL	heparin			inhibits					FGF 		signaling of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_340_s_152	14670838	15 Heparin inhibits FGF signaling by competing with HSPGs for binding bFGF. 15,28  Our data suggest that bFGF is released from the cells after stimulation with thrombin and FXa and binds to HSPGs in the pericellular matrix ( Figures 4A and 5   ).	bind
18862	5	6686	6	NULL	NULL	0	NULL	statement 4	NULL		occurs by	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_3_340_s_152	14670838	15 Heparin inhibits FGF signaling by competing with HSPGs for binding bFGF. 15,28  Our data suggest that bFGF is released from the cells after stimulation with thrombin and FXa and binds to HSPGs in the pericellular matrix ( Figures 4A and 5   ).	bind
18863	6	6686	6	NULL	NULL	0	NULL	bFGF	NULL		released from	NULL				cells	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_3_340_s_152	14670838	15 Heparin inhibits FGF signaling by competing with HSPGs for binding bFGF. 15,28  Our data suggest that bFGF is released from the cells after stimulation with thrombin and FXa and binds to HSPGs in the pericellular matrix ( Figures 4A and 5   ).	bind
18864	7	6686	6	NULL	NULL	0	NULL	statement 6	NULL		occurs after stimulation with	NULL				thrombin	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_3_340_s_152	14670838	15 Heparin inhibits FGF signaling by competing with HSPGs for binding bFGF. 15,28  Our data suggest that bFGF is released from the cells after stimulation with thrombin and FXa and binds to HSPGs in the pericellular matrix ( Figures 4A and 5   ).	bind
18865	8	6686	6	NULL	NULL	0	NULL	statement 6	NULL		occurs after stimulation with	NULL				FXa	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_3_340_s_152	14670838	15 Heparin inhibits FGF signaling by competing with HSPGs for binding bFGF. 15,28  Our data suggest that bFGF is released from the cells after stimulation with thrombin and FXa and binds to HSPGs in the pericellular matrix ( Figures 4A and 5   ).	bind
56352	9	6686	6	10	NULL	0	NULL	statement 7			occur along with					statement 8					NULL		0	NULL	NULL	NULL	gw70_circulationres_94_3_340_s_152	14670838	15 Heparin inhibits FGF signaling by competing with HSPGs for binding bFGF. 15,28  Our data suggest that bFGF is released from the cells after stimulation with thrombin and FXa and binds to HSPGs in the pericellular matrix ( Figures 4A and 5   ).	bind
56354	10	6686	6	10	NULL	0	NULL	statement 1			occurs after					statement 9					NULL		0	NULL	NULL	NULL	gw70_circulationres_94_3_340_s_152	14670838	15 Heparin inhibits FGF signaling by competing with HSPGs for binding bFGF. 15,28  Our data suggest that bFGF is released from the cells after stimulation with thrombin and FXa and binds to HSPGs in the pericellular matrix ( Figures 4A and 5   ).	bind
22925	1	6687	5	13	NULL	NULL	NULL	ADP-P2y12	GP		activates					type 1B PI3-K	GP				NULL	in human platelets	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_2_417_s_30	16339499	15 In human platelets, the role of type 1B PI3-K is less well understood, because although being activated by ADP-P2y12 contact, it appears under negative control by ADP-P2y1 binding and activation of Src and PKC. 10,16	bind
24809	2	6687	5	13	NULL	NULL	NULL	ADP-P2y1	GP	binding of	controls		negatively			type 1B PI3-K	GP				NULL	in human platelets	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_2_417_s_30	16339499	15 In human platelets, the role of type 1B PI3-K is less well understood, because although being activated by ADP-P2y12 contact, it appears under negative control by ADP-P2y1 binding and activation of Src and PKC. 10,16	bind
24810	3	6687	5	13	NULL	NULL	NULL	Src	GP	activation of	controls		negatively			type 1B PI3-K	GP				NULL	in human platelets	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_2_417_s_30	16339499	15 In human platelets, the role of type 1B PI3-K is less well understood, because although being activated by ADP-P2y12 contact, it appears under negative control by ADP-P2y1 binding and activation of Src and PKC. 10,16	bind
24811	4	6687	5	13	NULL	NULL	NULL	PKC	GP	activation of	controls		negatively			type 1B PI3-K	GP				NULL	in human platelets	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_2_417_s_30	16339499	15 In human platelets, the role of type 1B PI3-K is less well understood, because although being activated by ADP-P2y12 contact, it appears under negative control by ADP-P2y1 binding and activation of Src and PKC. 10,16	bind
18866	1	6687	6	NULL	NULL	0	NULL	type 1B PI3-K	NULL		is activated by	NULL				ADP-P2y12	NULL				NULL	human platelets	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_2_417_s_30	16339499	15 In human platelets, the role of type 1B PI3-K is less well understood, because although being activated by ADP-P2y12 contact, it appears under negative control by ADP-P2y1 binding and activation of Src and PKC. 10,16	bind
18867	2	6687	6	NULL	NULL	0	NULL	ADP-P2y12	NULL	binding of	controls	NULL	negatively 			type 1B PI3-K	NULL				NULL	human platelets	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_2_417_s_30	16339499	15 In human platelets, the role of type 1B PI3-K is less well understood, because although being activated by ADP-P2y12 contact, it appears under negative control by ADP-P2y1 binding and activation of Src and PKC. 10,16	bind
18868	3	6687	6	NULL	NULL	0	NULL	ADP-P2y12	NULL	binding of	controls	NULL	negatively			src	NULL	activation of			NULL	human platelets	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_2_417_s_30	16339499	15 In human platelets, the role of type 1B PI3-K is less well understood, because although being activated by ADP-P2y12 contact, it appears under negative control by ADP-P2y1 binding and activation of Src and PKC. 10,16	bind
18869	4	6687	6	NULL	NULL	0	NULL	ADP-P2y12	NULL	binding of	controls	NULL	negatively			PKC	NULL	activation of			NULL	human platelets	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_2_417_s_30	16339499	15 In human platelets, the role of type 1B PI3-K is less well understood, because although being activated by ADP-P2y12 contact, it appears under negative control by ADP-P2y1 binding and activation of Src and PKC. 10,16	bind
21788	1	6691	5	13	NULL	NULL	NULL	MyBP-C 	GP		bind					actin	GP				NULL	in solution	NULL	NULL	NULL	NULL	gw70_circulationres_93_8_752_s_133	14500336	15 MyBP-C also binds actin and regulated thin filaments in solution, and the latter is Ca2+ dependent.	bind
21789	2	6691	5	13	NULL	NULL	NULL	MyBP-C 	GP		bind					thin filaments	CellComponent	regulated			NULL	in solution	NULL	NULL	NULL	NULL	gw70_circulationres_93_8_752_s_133	14500336	15 MyBP-C also binds actin and regulated thin filaments in solution, and the latter is Ca2+ dependent.	bind
21790	3	6691	5	13	NULL	NULL	NULL	statement 2	Process		is dependent on					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_8_752_s_133	14500336	15 MyBP-C also binds actin and regulated thin filaments in solution, and the latter is Ca2+ dependent.	bind
18871	1	6691	6	10	NULL	0	NULL	MyBP-C			bind					actin					NULL	in solution	NULL	NULL	NULL	NULL	gw70_circulationres_93_8_752_s_133	14500336	15 MyBP-C also binds actin and regulated thin filaments in solution, and the latter is Ca2+ dependent.	bind
18872	2	6691	6	NULL	NULL	0	NULL	MyBP-C	NULL		regulates	NULL				thin filaments	NULL				NULL	in solution	0	NULL	NULL	NULL	gw70_circulationres_93_8_752_s_133	14500336	15 MyBP-C also binds actin and regulated thin filaments in solution, and the latter is Ca2+ dependent.	bind
18873	3	6691	6	NULL	NULL	0	NULL	statement 2	NULL		is dependent on	NULL				calcium	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_93_8_752_s_133	14500336	15 MyBP-C also binds actin and regulated thin filaments in solution, and the latter is Ca2+ dependent.	bind
21791	1	6692	5	13	NULL	NULL	NULL	Skp1	GP		bind					cdk2/cyclin A complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1217_s_165	15117732	15 Skp1 binds the cdk2/cyclin A complex and regulates the cell cycle by the timely destruction of numerous regulatory proteins such as cyclins.	bind
21793	2	6692	5	13	NULL	NULL	NULL	Skp1	GP		regulates					cell cycle	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1217_s_165	15117732	15 Skp1 binds the cdk2/cyclin A complex and regulates the cell cycle by the timely destruction of numerous regulatory proteins such as cyclins.	bind
21795	3	6692	5	13	NULL	NULL	NULL	Skp1	GP		destroys					regulatory proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1217_s_165	15117732	15 Skp1 binds the cdk2/cyclin A complex and regulates the cell cycle by the timely destruction of numerous regulatory proteins such as cyclins.	bind
21796	4	6692	5	13	NULL	NULL	NULL	statement 3	Process		is mechanism of					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1217_s_165	15117732	15 Skp1 binds the cdk2/cyclin A complex and regulates the cell cycle by the timely destruction of numerous regulatory proteins such as cyclins.	bind
18874	1	6692	6	NULL	NULL	0	NULL	Skp1	NULL		bind	NULL				cdk2/cyclin A complex	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1217_s_165	15117732	15 Skp1 binds the cdk2/cyclin A complex and regulates the cell cycle by the timely destruction of numerous regulatory proteins such as cyclins.	bind
18875	2	6692	6	NULL	NULL	0	NULL	Skp1	NULL		regulates	NULL				cell cycle	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1217_s_165	15117732	15 Skp1 binds the cdk2/cyclin A complex and regulates the cell cycle by the timely destruction of numerous regulatory proteins such as cyclins.	bind
30473	3	6692	6	NULL	NULL	0	NULL	Skp1	NULL		destroys	NULL				regulatory proteins	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1217_s_165	15117732	15 Skp1 binds the cdk2/cyclin A complex and regulates the cell cycle by the timely destruction of numerous regulatory proteins such as cyclins.	bind
30474	4	6692	6	NULL	NULL	0	NULL	statement 3	NULL		is the mechanism for	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1217_s_165	15117732	15 Skp1 binds the cdk2/cyclin A complex and regulates the cell cycle by the timely destruction of numerous regulatory proteins such as cyclins.	bind
21797	1	6693	5	13	NULL	NULL	NULL	BS-1 lectin	GP	biotin-labeled 	bind					luminal surface of endothelial cells	Cell				NULL	 ear skin from wild-type mice	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2108_s_94	15345507	15 The architecture of the microvasculature was examined in whole-mount preparations of ear skin from wild-type and beta3-null mice in which vessels were visualized with biotin-labeled BS-1 lectin, which binds to the luminal surface of endothelial cells.	bind
21798	2	6693	5	13	NULL	NULL	NULL	BS-1 lectin	GP	biotin-labeled 	bind					luminal surface of endothelial cells	Cell				NULL	ear skin from beta3-null mice	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2108_s_94	15345507	15 The architecture of the microvasculature was examined in whole-mount preparations of ear skin from wild-type and beta3-null mice in which vessels were visualized with biotin-labeled BS-1 lectin, which binds to the luminal surface of endothelial cells.	bind
18879	1	6693	6	10	NULL	0	NULL	BS-1 lectin		biotin-labeled	bind					luminal surface of endothelial cells					NULL	ear skin from wild type mice	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2108_s_94	15345507	15 The architecture of the microvasculature was examined in whole-mount preparations of ear skin from wild-type and beta3-null mice in which vessels were visualized with biotin-labeled BS-1 lectin, which binds to the luminal surface of endothelial cells.	bind
18880	2	6693	6	10	NULL	0	NULL	BS-1 lectin		biotin-labeled	bind					luminal surface of endothelial cells					NULL	ear skin from beta3-null mice	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2108_s_94	15345507	15 The architecture of the microvasculature was examined in whole-mount preparations of ear skin from wild-type and beta3-null mice in which vessels were visualized with biotin-labeled BS-1 lectin, which binds to the luminal surface of endothelial cells.	bind
21799	1	6694	5	13	NULL	NULL	NULL	E-cadherin	GP		is different from			p120ctn binding site		E-cadherin	GP		beta- catenin/plakoglobin binding site		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_3_787_s_21	10487836	15 The p120ctn binding site in E-cadherin is different from the beta- catenin/plakoglobin binding site and p120ctn does not bind to alpha-catenin.	bind
21800	2	6694	5	13	NULL	NULL	NULL	p120ctn	GP		does not bind					alpha-catenin	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_3_787_s_21	10487836	15 The p120ctn binding site in E-cadherin is different from the beta- catenin/plakoglobin binding site and p120ctn does not bind to alpha-catenin.	bind
18882	1	6694	6	NULL	NULL	0	NULL	p120ctn	NULL		does not bind	NULL				alpha-catenin	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_3_787_s_21	10487836	15 The p120ctn binding site in E-cadherin is different from the beta- catenin/plakoglobin binding site and p120ctn does not bind to alpha-catenin.	bind
30533	2	6694	6	10	NULL	0	NULL	E-cadherin			is different from			p120ctn binding site		E-cadherin			beta- catenin/plakoglobin binding site		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_3_787_s_21	10487836	15 The p120ctn binding site in E-cadherin is different from the beta- catenin/plakoglobin binding site and p120ctn does not bind to alpha-catenin.	bind
21802	1	6696	5	13	NULL	NULL	NULL	CRP	GP		bind					FcgammaRI	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_109_21_2566_s_151	15136507	15 We found that blocking binding of CRP to FcgammaRI abolished the positive regulatory effect of CRP on monocyte CCR2 expression.	bind
21805	2	6696	5	13	NULL	NULL	NULL	CRP	GP		regulates		positive			CCR2	GP	expression of			NULL	monocyte	NULL	NULL	NULL	NULL	gw70_circulation_109_21_2566_s_151	15136507	15 We found that blocking binding of CRP to FcgammaRI abolished the positive regulatory effect of CRP on monocyte CCR2 expression.	bind
21806	3	6696	5	13	NULL	NULL	NULL	statement 1	Process	blocking of	abolishes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_109_21_2566_s_151	15136507	15 We found that blocking binding of CRP to FcgammaRI abolished the positive regulatory effect of CRP on monocyte CCR2 expression.	bind
18906	1	6696	6	NULL	NULL	0	NULL	CRP	NULL		bind	NULL				FcgammaRI	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_109_21_2566_s_151	15136507	15 We found that blocking binding of CRP to FcgammaRI abolished the positive regulatory effect of CRP on monocyte CCR2 expression.	bind
18908	2	6696	6	NULL	NULL	0	NULL	CRP	NULL		regulates	NULL	positively			CCR2 	NULL	expression of			NULL	monocytes	NULL	NULL	NULL	NULL	gw70_circulation_109_21_2566_s_151	15136507	15 We found that blocking binding of CRP to FcgammaRI abolished the positive regulatory effect of CRP on monocyte CCR2 expression.	bind
18910	3	6696	6	NULL	NULL	0	NULL	statement 1	NULL	blocking of	abolishes	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_109_21_2566_s_151	15136507	15 We found that blocking binding of CRP to FcgammaRI abolished the positive regulatory effect of CRP on monocyte CCR2 expression.	bind
21824	1	6697	5	13	NULL	NULL	NULL	P. aeruginosa	Organism		induces					MUC2	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_4_1475_s_268	12368220	15, 16  MUC2 transcription induced by  P. aeruginosa was mediated by the binding of NF-kappaB (p55 and p65 subunits) to this kappaB site.	bind
21825	2	6697	5	13	NULL	NULL	NULL	NF-kappaB	GP		bind									kappaB site	NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_4_1475_s_268	12368220	15, 16  MUC2 transcription induced by  P. aeruginosa was mediated by the binding of NF-kappaB (p55 and p65 subunits) to this kappaB site.	bind
21826	3	6697	5	13	NULL	NULL	NULL	NF-kappaB	GP		consists of					p55 subunit	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_4_1475_s_268	12368220	15, 16  MUC2 transcription induced by  P. aeruginosa was mediated by the binding of NF-kappaB (p55 and p65 subunits) to this kappaB site.	bind
21827	4	6697	5	13	NULL	NULL	NULL	NF-kappaB	GP		consists of					p65 subunit	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_4_1475_s_268	12368220	15, 16  MUC2 transcription induced by  P. aeruginosa was mediated by the binding of NF-kappaB (p55 and p65 subunits) to this kappaB site.	bind
21828	5	6697	5	13	NULL	NULL	NULL	statement 2	Process		mediate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_4_1475_s_268	12368220	15, 16  MUC2 transcription induced by  P. aeruginosa was mediated by the binding of NF-kappaB (p55 and p65 subunits) to this kappaB site.	bind
19000	1	6697	6	NULL	NULL	0	NULL	MUC2	NULL	transcription of	is induced by	NULL				P. aeruginosa	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_4_1475_s_268	12368220	15, 16  MUC2 transcription induced by  P. aeruginosa was mediated by the binding of NF-kappaB (p55 and p65 subunits) to this kappaB site.	bind
19004	2	6697	6	NULL	NULL	0	NULL	NF-kappaB	NULL		bind	NULL					NULL			kappaB site	NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_4_1475_s_268	12368220	15, 16  MUC2 transcription induced by  P. aeruginosa was mediated by the binding of NF-kappaB (p55 and p65 subunits) to this kappaB site.	bind
19005	3	6697	6	NULL	NULL	0	NULL	statement 1	NULL		is mediated by	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_4_1475_s_268	12368220	15, 16  MUC2 transcription induced by  P. aeruginosa was mediated by the binding of NF-kappaB (p55 and p65 subunits) to this kappaB site.	bind
56355	4	6697	6	10	NULL	0	NULL	NF-kappaB			consist of					p55 subunit					NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_4_1475_s_268	12368220	15, 16  MUC2 transcription induced by  P. aeruginosa was mediated by the binding of NF-kappaB (p55 and p65 subunits) to this kappaB site.	bind
56356	5	6697	6	10	NULL	0	NULL	NF-kappaB			consist of					p65 subunit					NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_4_1475_s_268	12368220	15, 16  MUC2 transcription induced by  P. aeruginosa was mediated by the binding of NF-kappaB (p55 and p65 subunits) to this kappaB site.	bind
21829	1	6698	5	13	NULL	NULL	NULL				upstream of				kappaB-binding site	MUC2 gene	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_4_1475_s_267	12368220	15, 16, 41  The kappaB-binding site exists upstream of the MUC2 gene, which can bind to a transcription factor, nuclear factor (NF)-kappaB.	bind
21830	2	6698	5	13	NULL	NULL	NULL	MUC2 gene	GP		bind				kappaB-binding site	NF-kappaB	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_4_1475_s_267	12368220	15, 16, 41  The kappaB-binding site exists upstream of the MUC2 gene, which can bind to a transcription factor, nuclear factor (NF)-kappaB.	bind
21831	3	6698	5	13	NULL	NULL	NULL	NF-kappaB	GP		is					nuclear factor-kappaB	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_4_1475_s_267	12368220	15, 16, 41  The kappaB-binding site exists upstream of the MUC2 gene, which can bind to a transcription factor, nuclear factor (NF)-kappaB.	bind
19008	1	6698	6	NULL	NULL	0	NULL	NF-kappaB	NULL		bind	NULL				MUC2 gene	NULL			kappaB-binding site	NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_4_1475_s_267	12368220	15, 16, 41  The kappaB-binding site exists upstream of the MUC2 gene, which can bind to a transcription factor, nuclear factor (NF)-kappaB.	bind
30534	2	6698	6	NULL	NULL	0	NULL		NULL		exists	NULL			kappaB-binding site	MUC2 gene	NULL	upstream of 			NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_4_1475_s_267	12368220	15, 16, 41  The kappaB-binding site exists upstream of the MUC2 gene, which can bind to a transcription factor, nuclear factor (NF)-kappaB.	bind
30535	3	6698	6	NULL	NULL	0	NULL	NF-kappaB	NULL		is	NULL				nuclear factor-kappaB	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_4_1475_s_267	12368220	15, 16, 41  The kappaB-binding site exists upstream of the MUC2 gene, which can bind to a transcription factor, nuclear factor (NF)-kappaB.	bind
21832	1	6699	5	13	NULL	NULL	NULL	XIP	GP	exogenous	bind		avidly			PIP2	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_1_91_s_177	15550690	15,16  Because exogenous XIP also avidly binds to PIP2, 15 it may be speculated that differences in the native membrane content of PIP2 between cardiac myocytes, HEK, and A549 cells may also account for the different inhibitory efficacy of XIP in these cells.	bind
19009	1	6699	6	NULL	NULL	0	NULL	XIP	NULL	exogenous	bind	NULL	avidly			PIP2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_1_91_s_177	15550690	15,16  Because exogenous XIP also avidly binds to PIP2, 15 it may be speculated that differences in the native membrane content of PIP2 between cardiac myocytes, HEK, and A549 cells may also account for the different inhibitory efficacy of XIP in these cells.	bind
21833	1	6700	5	13	NULL	NULL	NULL	decorin	GP		bind					TGF-beta 17	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_163_3_869_s_17	12937128	15,16  It is well established that decorin binds to TGF-beta 17  and inhibits its biological activity in a number of cell types, including rat aortic SMCs. 16  However, it is not known whether decorin may also exert its regulatory effects by interacting with and modulating the activity of PDGF, another prominent growth factor involved in arterial repair.	bind
21834	2	6700	5	13	NULL	NULL	NULL	statement 1	Process		inhibit					TGF-beta 17	GP	biological activity of			NULL	in a number of cell types, including rat aortic SMCs	NULL	NULL	NULL	NULL	gw60_amjpathol_163_3_869_s_17	12937128	15,16  It is well established that decorin binds to TGF-beta 17  and inhibits its biological activity in a number of cell types, including rat aortic SMCs. 16  However, it is not known whether decorin may also exert its regulatory effects by interacting with and modulating the activity of PDGF, another prominent growth factor involved in arterial repair.	bind
19051	1	6700	6	NULL	NULL	0	NULL	decorin	NULL		bind	NULL				TGF-beta17	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_163_3_869_s_17	12937128	15,16  It is well established that decorin binds to TGF-beta 17  and inhibits its biological activity in a number of cell types, including rat aortic SMCs. 16  However, it is not known whether decorin may also exert its regulatory effects by interacting with and modulating the activity of PDGF, another prominent growth factor involved in arterial repair.	bind
19052	2	6700	6	NULL	NULL	0	NULL	statement 1	NULL		inhibits	NULL				TGF-beta17	NULL	biological activity of			NULL	rat aortic SMCs	NULL	NULL	NULL	NULL	gw60_amjpathol_163_3_869_s_17	12937128	15,16  It is well established that decorin binds to TGF-beta 17  and inhibits its biological activity in a number of cell types, including rat aortic SMCs. 16  However, it is not known whether decorin may also exert its regulatory effects by interacting with and modulating the activity of PDGF, another prominent growth factor involved in arterial repair.	bind
21835	1	6701	5	13	NULL	NULL	NULL	p65 NF-kappaB	GP		bind					ICAM-1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_41_s_132	14551154	15,37  PKC-delta was also implicated in thrombin-mediated induction of p65 NF-kappaB binding to the ICAM-1 promoter.	bind
21836	2	6701	5	13	NULL	NULL	NULL	statement 1	Process	induction of	is mediated by					thrombin	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_41_s_132	14551154	15,37  PKC-delta was also implicated in thrombin-mediated induction of p65 NF-kappaB binding to the ICAM-1 promoter.	bind
21837	3	6701	5	13	NULL	NULL	NULL	PKC-delta	GP		is implicated in					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_41_s_132	14551154	15,37  PKC-delta was also implicated in thrombin-mediated induction of p65 NF-kappaB binding to the ICAM-1 promoter.	bind
19088	1	6701	6	NULL	NULL	0	NULL	p65 NF-kappaB	NULL		bind	NULL				ICAM-1	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_41_s_132	14551154	15,37  PKC-delta was also implicated in thrombin-mediated induction of p65 NF-kappaB binding to the ICAM-1 promoter.	bind
19089	2	6701	6	NULL	NULL	0	NULL	thrombin	NULL		mediates	NULL				statement 1	NULL	induction of 			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_41_s_132	14551154	15,37  PKC-delta was also implicated in thrombin-mediated induction of p65 NF-kappaB binding to the ICAM-1 promoter.	bind
56458	3	6701	6	10	NULL	0	NULL	PKC-delta			is implicated in					statement 2					NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_41_s_132	14551154	15,37  PKC-delta was also implicated in thrombin-mediated induction of p65 NF-kappaB binding to the ICAM-1 promoter.	bind
21838	1	6702	5	13	NULL	NULL	NULL	NF-kappaB	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_16_10863_s_330	10196163	15-Deoxy-Delta 12,14-prostaglandin J2 Inhibition of NF-kappa B-DNA Binding through Covalent Modification of the p50 Subunit.	bind
21839	2	6702	5	13	NULL	NULL	NULL	15-Deoxy-Delta 12,14-prostaglandin J2	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_16_10863_s_330	10196163	15-Deoxy-Delta 12,14-prostaglandin J2 Inhibition of NF-kappa B-DNA Binding through Covalent Modification of the p50 Subunit.	bind
21840	3	6702	5	13	NULL	NULL	NULL	statement 2	Process		occurs through					p50 Subunit	GP	covalent modification of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_16_10863_s_330	10196163	15-Deoxy-Delta 12,14-prostaglandin J2 Inhibition of NF-kappa B-DNA Binding through Covalent Modification of the p50 Subunit.	bind
19090	1	6702	6	NULL	NULL	0	NULL	NF-kappaB	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_16_10863_s_330	10196163	15-Deoxy-Delta 12,14-prostaglandin J2 Inhibition of NF-kappa B-DNA Binding through Covalent Modification of the p50 Subunit.	bind
19091	2	6702	6	NULL	NULL	0	NULL	15-Deoxy-Delta 12,14-prostaglandin J2	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_16_10863_s_330	10196163	15-Deoxy-Delta 12,14-prostaglandin J2 Inhibition of NF-kappa B-DNA Binding through Covalent Modification of the p50 Subunit.	bind
19152	3	6702	6	NULL	NULL	0	NULL	statement 2	NULL		occurs via	NULL				p50 subuit	NULL	covalent modification of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_16_10863_s_330	10196163	15-Deoxy-Delta 12,14-prostaglandin J2 Inhibition of NF-kappa B-DNA Binding through Covalent Modification of the p50 Subunit.	bind
21848	1	6704	5	13	NULL	NULL	NULL	15-deoxy-delta12,14-PGJ2	Chemical		is					PGD2 metabolite	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_137_8_1163_s_205	12466225	15-deoxy-delta12,14-PGJ2 is another PGD2 metabolite which preferentially binds CRTH2 over DP with 89 fold selectivity.	bind
21849	2	6704	5	13	NULL	NULL	NULL	15-deoxy-delta12,14-PGJ2	Chemical		bind		preferentially			CRTH2	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_137_8_1163_s_205	12466225	15-deoxy-delta12,14-PGJ2 is another PGD2 metabolite which preferentially binds CRTH2 over DP with 89 fold selectivity.	bind
21851	3	6704	5	13	NULL	NULL	NULL	15-deoxy-delta12,14-PGJ2	Chemical		bind					DP	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_137_8_1163_s_205	12466225	15-deoxy-delta12,14-PGJ2 is another PGD2 metabolite which preferentially binds CRTH2 over DP with 89 fold selectivity.	bind
21852	4	6704	5	13	NULL	NULL	NULL	statement 2	Process		is prefered over					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_137_8_1163_s_205	12466225	15-deoxy-delta12,14-PGJ2 is another PGD2 metabolite which preferentially binds CRTH2 over DP with 89 fold selectivity.	bind
19153	1	6704	6	NULL	NULL	0	NULL	15-deoxy-delta12,14-PGJ2	NULL		is	NULL				PGD2 metabolite	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_137_8_1163_s_205	12466225	15-deoxy-delta12,14-PGJ2 is another PGD2 metabolite which preferentially binds CRTH2 over DP with 89 fold selectivity.	bind
19173	2	6704	6	NULL	NULL	0	NULL	15-deoxy-delta12,14-PGJ2	NULL		bind	NULL	preferentially			CRTH2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_137_8_1163_s_205	12466225	15-deoxy-delta12,14-PGJ2 is another PGD2 metabolite which preferentially binds CRTH2 over DP with 89 fold selectivity.	bind
19174	3	6704	6	NULL	NULL	0	NULL	15-deoxy-delta12,14-PGJ2	NULL		bind	NULL				DP	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_137_8_1163_s_205	12466225	15-deoxy-delta12,14-PGJ2 is another PGD2 metabolite which preferentially binds CRTH2 over DP with 89 fold selectivity.	bind
19175	4	6704	6	NULL	NULL	0	NULL	statement 2	NULL		is more preferential than	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_137_8_1163_s_205	12466225	15-deoxy-delta12,14-PGJ2 is another PGD2 metabolite which preferentially binds CRTH2 over DP with 89 fold selectivity.	bind
21861	1	6706	5	13	NULL	NULL	NULL	15/7	GP		enhances					cell adhesion	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_48_28740_s_289	7499396	15/7 Enhances Cell Adhesion by Stabilizing an Active  Conformation of beta  Integrin15/7  promoted THP-1 cell binding to beta   integrin ligands, even  though the cells did not express a significant level of the 15/7  epitope ( Fig. 5).	bind
21862	2	6706	5	13	NULL	NULL	NULL	15/7	GP		stabilizes					beta Integrin	GP	active conformation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_48_28740_s_289	7499396	15/7 Enhances Cell Adhesion by Stabilizing an Active  Conformation of beta  Integrin15/7  promoted THP-1 cell binding to beta   integrin ligands, even  though the cells did not express a significant level of the 15/7  epitope ( Fig. 5).	bind
21863	3	6706	5	13	NULL	NULL	NULL	statement 2	Process		leads to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_48_28740_s_289	7499396	15/7 Enhances Cell Adhesion by Stabilizing an Active  Conformation of beta  Integrin15/7  promoted THP-1 cell binding to beta   integrin ligands, even  though the cells did not express a significant level of the 15/7  epitope ( Fig. 5).	bind
21864	4	6706	5	13	NULL	NULL	NULL	THP-1 cell	Cell		bind					beta integrin ligands	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_48_28740_s_289	7499396	15/7 Enhances Cell Adhesion by Stabilizing an Active  Conformation of beta  Integrin15/7  promoted THP-1 cell binding to beta   integrin ligands, even  though the cells did not express a significant level of the 15/7  epitope ( Fig. 5).	bind
21865	5	6706	5	13	NULL	NULL	NULL	15/7	GP		promote					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_48_28740_s_289	7499396	15/7 Enhances Cell Adhesion by Stabilizing an Active  Conformation of beta  Integrin15/7  promoted THP-1 cell binding to beta   integrin ligands, even  though the cells did not express a significant level of the 15/7  epitope ( Fig. 5).	bind
56462	6	6706	5	13	NULL	NULL	NULL	THP-1 cell 	Cell		does not express					15/7 epitope	GP	significant level of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_48_28740_s_289	7499396	15/7 Enhances Cell Adhesion by Stabilizing an Active  Conformation of beta  Integrin15/7  promoted THP-1 cell binding to beta   integrin ligands, even  though the cells did not express a significant level of the 15/7  epitope ( Fig. 5).	bind
19446	1	6706	6	NULL	NULL	0	NULL	THP-1 cell	NULL		bind	NULL				beta integrin ligands	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_48_28740_s_289	7499396	15/7 Enhances Cell Adhesion by Stabilizing an Active  Conformation of beta  Integrin15/7  promoted THP-1 cell binding to beta   integrin ligands, even  though the cells did not express a significant level of the 15/7  epitope ( Fig. 5).	bind
19447	2	6706	6	10	NULL	0	NULL	15/7			promotes					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_48_28740_s_289	7499396	15/7 Enhances Cell Adhesion by Stabilizing an Active  Conformation of beta  Integrin15/7  promoted THP-1 cell binding to beta   integrin ligands, even  though the cells did not express a significant level of the 15/7  epitope ( Fig. 5).	bind
19448	3	6706	6	10	NULL	0	NULL	THP-1 cells			does not express					15/7 epitope		significant level of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_48_28740_s_289	7499396	15/7 Enhances Cell Adhesion by Stabilizing an Active  Conformation of beta  Integrin15/7  promoted THP-1 cell binding to beta   integrin ligands, even  though the cells did not express a significant level of the 15/7  epitope ( Fig. 5).	bind
56459	4	6706	6	10	NULL	0	NULL	15/7			enhance					cell adhesion					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_48_28740_s_289	7499396	15/7 Enhances Cell Adhesion by Stabilizing an Active  Conformation of beta  Integrin15/7  promoted THP-1 cell binding to beta   integrin ligands, even  though the cells did not express a significant level of the 15/7  epitope ( Fig. 5).	bind
56460	5	6706	6	10	NULL	0	NULL	15/7			stabilize					beta Integrin		active conformation of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_48_28740_s_289	7499396	15/7 Enhances Cell Adhesion by Stabilizing an Active  Conformation of beta  Integrin15/7  promoted THP-1 cell binding to beta   integrin ligands, even  though the cells did not express a significant level of the 15/7  epitope ( Fig. 5).	bind
56461	6	6706	6	10	NULL	0	NULL	statement 1			occur by					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_48_28740_s_289	7499396	15/7 Enhances Cell Adhesion by Stabilizing an Active  Conformation of beta  Integrin15/7  promoted THP-1 cell binding to beta   integrin ligands, even  though the cells did not express a significant level of the 15/7  epitope ( Fig. 5).	bind
21866	1	6708	5	13	NULL	NULL	NULL	H4	GP	acetylation	occurs at					 eotaxin	GP			promoter	NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
21867	2	6708	5	13	NULL	NULL	NULL	TNFalpha	GP		induces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
21868	3	6708	5	13	NULL	NULL	NULL	15d-PGJ(2)	Chemical		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
21869	4	6708	5	13	NULL	NULL	NULL	fluticasone	Chemical		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
21870	5	6708	5	13	NULL	NULL	NULL	salmeterol	Chemical		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
21871	6	6708	5	13	NULL	NULL	NULL	NF-kappaB p65	GP		bind					eotaxin	GP			promoter	NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
21872	7	6708	5	13	NULL	NULL	NULL	15d-PGJ(2)	Chemical		inhibit					statement 6	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
21873	8	6708	5	13	NULL	NULL	NULL	fluticasone	Chemical		inhibit					statement 6	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
21874	9	6708	5	13	NULL	NULL	NULL	salmeterol	Chemical		inhibit					statement 6	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
21875	10	6708	5	13	NULL	NULL	NULL	PPARgamma	GP		associates with					eotaxin	GP			promoter	NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
21876	11	6708	5	13	NULL	NULL	NULL	15d-PGJ(2)	Chemical		induces					statement 10	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
21877	12	6708	5	13	NULL	NULL	NULL	fluticasone	Chemical		induces					statement 10	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
21878	13	6708	5	13	NULL	NULL	NULL	salmeterol	Chemical		induces					statement 10	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
21879	14	6708	5	13	NULL	NULL	NULL	GR	GP		associates with					eotaxin	GP			promoter	NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
21880	15	6708	5	13	NULL	NULL	NULL	15d-PGJ(2)	Chemical		induces					statement 14	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
21881	16	6708	5	13	NULL	NULL	NULL	fluticasone	Chemical		induces					statement 14	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
21882	17	6708	5	13	NULL	NULL	NULL	salmeterol	Chemical		induces					statement 14	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
19449	1	6708	6	NULL	NULL	0	NULL	NF-kappaB p65	NULL		bind	NULL				eotaxin	NULL			promoter	NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
19450	2	6708	6	NULL	NULL	0	NULL	histone H4	NULL		acetylated at	NULL				eotaxin	NULL			promoter	NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
19451	3	6708	6	NULL	NULL	0	NULL	TNF-alpha	NULL		induces	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
19452	4	6708	6	NULL	NULL	0	NULL	PPARgamma	NULL		associates with	NULL				eotaxin 	NULL			promoter	NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
19453	5	6708	6	NULL	NULL	0	NULL	GR	NULL		associates with	NULL				eotaxin	NULL			promoter	NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
19454	6	6708	6	NULL	NULL	0	NULL	15d-PGJ(2)	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
19455	7	6708	6	NULL	NULL	0	NULL	15d-PGJ(2)	NULL		inhibits	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
19456	8	6708	6	NULL	NULL	0	NULL	15d-PGJ(2)	NULL		induces	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
19457	9	6708	6	NULL	NULL	0	NULL	15d-PGJ(2)	NULL		induces	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
19458	10	6708	6	NULL	NULL	0	NULL	fluticasone	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
19459	11	6708	6	NULL	NULL	0	NULL	fluticasone	NULL		inhibits	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
19460	12	6708	6	NULL	NULL	0	NULL	fluticasone	NULL		induces	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
19461	13	6708	6	NULL	NULL	0	NULL	fluticasone	NULL		induces	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
19462	14	6708	6	NULL	NULL	0	NULL	salmeterol	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
19463	15	6708	6	NULL	NULL	0	NULL	salmeterol	NULL		inhibits	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
19464	16	6708	6	NULL	NULL	0	NULL	salmeterol	NULL		induces	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
19465	17	6708	6	NULL	NULL	0	NULL	salmeterol	NULL		induces	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_280_4_15531761_s_8	15531761	15d-PGJ(2), fluticasone, and  salmeterol all inhibited TNFalpha-induced histone H4 acetylation at the  eotaxin promoter and NF-kappaB p65 binding to the eotaxin promoter and  induced PPARgamma and GR association with the eotaxin promoter, as analyzed  by chromatin immunoprecipitation assay.	bind
21844	1	6709	5	13	NULL	NULL	NULL	p300	GP		bind					PPARgamma	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_9_3057_s_204	11287611	15d-PGJ2 enhanced binding of p300 to PPARgamma and reduced binding to c-Fos.	bind
21845	2	6709	5	13	NULL	NULL	NULL	15d-PGJ2	Chemical		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_9_3057_s_204	11287611	15d-PGJ2 enhanced binding of p300 to PPARgamma and reduced binding to c-Fos.	bind
21846	3	6709	5	13	NULL	NULL	NULL	p300	GP		bind					c-Fos	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_9_3057_s_204	11287611	15d-PGJ2 enhanced binding of p300 to PPARgamma and reduced binding to c-Fos.	bind
21847	4	6709	5	13	NULL	NULL	NULL	15d-PGJ2	Chemical		reduces					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_9_3057_s_204	11287611	15d-PGJ2 enhanced binding of p300 to PPARgamma and reduced binding to c-Fos.	bind
19177	1	6709	6	NULL	NULL	0	NULL	p300	NULL		bind	NULL				PPARgamma	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_9_3057_s_204	11287611	15d-PGJ2 enhanced binding of p300 to PPARgamma and reduced binding to c-Fos.	bind
19178	2	6709	6	NULL	NULL	0	NULL	p300	NULL		bind	NULL				c-Fos	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_9_3057_s_204	11287611	15d-PGJ2 enhanced binding of p300 to PPARgamma and reduced binding to c-Fos.	bind
19179	3	6709	6	NULL	NULL	0	NULL	15d-PGJ2	NULL		enhanced	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_9_3057_s_204	11287611	15d-PGJ2 enhanced binding of p300 to PPARgamma and reduced binding to c-Fos.	bind
19180	4	6709	6	NULL	NULL	0	NULL	15d-PGJ2	NULL		reduced	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_9_3057_s_204	11287611	15d-PGJ2 enhanced binding of p300 to PPARgamma and reduced binding to c-Fos.	bind
22116	1	6711	5	13	NULL	NULL	NULL	Tbeta4	GP		bind			Leu		G-actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_22_23637_s_198	15039431	15N HSQC spectra of [15]AA Tbeta4 (where AA is Leu, Thr, or Lys) bound to G-actin are shown in  Fig. 3 B. Resonances obtained for the selectively labeled Tbeta4 perfectly superimposed those obtained for the uniformly labeled protein.	bind
22117	2	6711	5	13	NULL	NULL	NULL	Tbeta4	GP		bind			Thr		G-actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_22_23637_s_198	15039431	15N HSQC spectra of [15]AA Tbeta4 (where AA is Leu, Thr, or Lys) bound to G-actin are shown in  Fig. 3 B. Resonances obtained for the selectively labeled Tbeta4 perfectly superimposed those obtained for the uniformly labeled protein.	bind
22118	3	6711	5	13	NULL	NULL	NULL	Tbeta4	GP		bind			Lys		G-actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_22_23637_s_198	15039431	15N HSQC spectra of [15]AA Tbeta4 (where AA is Leu, Thr, or Lys) bound to G-actin are shown in  Fig. 3 B. Resonances obtained for the selectively labeled Tbeta4 perfectly superimposed those obtained for the uniformly labeled protein.	bind
19181	1	6711	6	NULL	NULL	0	NULL	Tbeta4	NULL		bind	NULL		Leu		G-actin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_22_23637_s_198	15039431	15N HSQC spectra of [15]AA Tbeta4 (where AA is Leu, Thr, or Lys) bound to G-actin are shown in  Fig. 3 B. Resonances obtained for the selectively labeled Tbeta4 perfectly superimposed those obtained for the uniformly labeled protein.	bind
19182	2	6711	6	NULL	NULL	0	NULL	Tbeta4	NULL		bind	NULL		Thr		G-actin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_22_23637_s_198	15039431	15N HSQC spectra of [15]AA Tbeta4 (where AA is Leu, Thr, or Lys) bound to G-actin are shown in  Fig. 3 B. Resonances obtained for the selectively labeled Tbeta4 perfectly superimposed those obtained for the uniformly labeled protein.	bind
19183	3	6711	6	NULL	NULL	0	NULL	Tbeta4	NULL		bind	NULL		Lys		G-actin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_22_23637_s_198	15039431	15N HSQC spectra of [15]AA Tbeta4 (where AA is Leu, Thr, or Lys) bound to G-actin are shown in  Fig. 3 B. Resonances obtained for the selectively labeled Tbeta4 perfectly superimposed those obtained for the uniformly labeled protein.	bind
22119	1	6712	5	13	NULL	NULL	NULL	cTnC	GP	Ca2+ saturated	bind					cTnI	GP		1-80		NULL		NULL	NULL	NULL	NULL	gw60_febslett_469_2_168_s_142	10713265	15{1} heteronuclear NOE values for Ca2+ saturated [15N, 2]cTnC bound to cTnI(1-80)	bind
19184	1	6712	6	10	NULL	0	NULL	cTnC	NULL	Ca2+ saturated	bind	NULL				cTnI	NULL		1-80		NULL		NULL	NULL	NULL	NULL	gw60_febslett_469_2_168_s_142	10713265	15{1} heteronuclear NOE values for Ca2+ saturated [15N, 2]cTnC bound to cTnI(1-80)	bind
22120	1	6714	5	13	NULL	NULL	NULL	CBF1	GP		belongs to					helix - loophelix protein family	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_5_1054_s_247	11222754	16       Cai,M. and Davis,R.W. (1990) Yeast centromere binding protein CBF1, of the  - helix - loophelix protein family, is required for chromosome stability and methionine prototrophy.	bind
22121	2	6714	5	13	NULL	NULL	NULL	CBF1	GP		is					Yeast centromere binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_5_1054_s_247	11222754	16       Cai,M. and Davis,R.W. (1990) Yeast centromere binding protein CBF1, of the  - helix - loophelix protein family, is required for chromosome stability and methionine prototrophy.	bind
22122	3	6714	5	13	NULL	NULL	NULL	CBF1	GP		is required for					chromosome	Chromosome	stability of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_5_1054_s_247	11222754	16       Cai,M. and Davis,R.W. (1990) Yeast centromere binding protein CBF1, of the  - helix - loophelix protein family, is required for chromosome stability and methionine prototrophy.	bind
22123	4	6714	5	13	NULL	NULL	NULL	CBF1	GP		is required for					methionine prototrophy	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_5_1054_s_247	11222754	16       Cai,M. and Davis,R.W. (1990) Yeast centromere binding protein CBF1, of the  - helix - loophelix protein family, is required for chromosome stability and methionine prototrophy.	bind
19185	1	6714	6	NULL	NULL	0	NULL	CBF1	NULL		is	NULL				centromere binding protein	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_5_1054_s_247	11222754	16       Cai,M. and Davis,R.W. (1990) Yeast centromere binding protein CBF1, of the  - helix - loophelix protein family, is required for chromosome stability and methionine prototrophy.	bind
19186	2	6714	6	NULL	NULL	0	NULL	CBF1	NULL	yeast	is a member of	NULL				helix - loophelix protein family	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_5_1054_s_247	11222754	16       Cai,M. and Davis,R.W. (1990) Yeast centromere binding protein CBF1, of the  - helix - loophelix protein family, is required for chromosome stability and methionine prototrophy.	bind
19187	3	6714	6	10	NULL	0	NULL	CBF1		yeast	is required for					chromosome 		stability of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_5_1054_s_247	11222754	16       Cai,M. and Davis,R.W. (1990) Yeast centromere binding protein CBF1, of the  - helix - loophelix protein family, is required for chromosome stability and methionine prototrophy.	bind
19188	4	6714	6	NULL	NULL	0	NULL	CBF1	NULL	yeast	is required for	NULL				methionine prototrophy	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_5_1054_s_247	11222754	16       Cai,M. and Davis,R.W. (1990) Yeast centromere binding protein CBF1, of the  - helix - loophelix protein family, is required for chromosome stability and methionine prototrophy.	bind
22124	1	6715	5	13	NULL	NULL	NULL	HAP1	GP		bind		dramatically;;assymetrically			DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_10_2181_s_237	11353088	16       King,D.A., Zhang,L., Guarente,L. and Marmorstein,R. (1999) Structure of a HAP1 - DNA complex reveals dramatically asymmetric DNA binding by a homodimeric protein.	bind
56497	2	6715	5	13	NULL	NULL	NULL	HAP1	GP		is a type of					homodimeric protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_10_2181_s_237	11353088	16       King,D.A., Zhang,L., Guarente,L. and Marmorstein,R. (1999) Structure of a HAP1 - DNA complex reveals dramatically asymmetric DNA binding by a homodimeric protein.	bind
19189	1	6715	6	10	NULL	0	NULL	HAP1			bind		dramatically;;assymetrically			DNA					NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_10_2181_s_237	11353088	16       King,D.A., Zhang,L., Guarente,L. and Marmorstein,R. (1999) Structure of a HAP1 - DNA complex reveals dramatically asymmetric DNA binding by a homodimeric protein.	bind
56498	2	6715	6	10	NULL	0	NULL	HAP1			is a type of					homodimeric protein					NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_10_2181_s_237	11353088	16       King,D.A., Zhang,L., Guarente,L. and Marmorstein,R. (1999) Structure of a HAP1 - DNA complex reveals dramatically asymmetric DNA binding by a homodimeric protein.	bind
22125	1	6716	5	13	NULL	NULL	NULL	RPA	GP		is					Replication Protein A	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_23_4634_s_289	11095672	16       Patrick,S.M. and Turchi,J.J. (1999) Replication Protein A (RPA) Binding to Duplex Cisplatin-Damaged DNA Is Mediated Through the Generation of Single-Stranded DNA.  J. Biol.	bind
22126	2	6716	5	13	NULL	NULL	NULL	RPA	GP		bind					duplex DNA	NucleicAcid	cisplatin-damaged			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_23_4634_s_289	11095672	16       Patrick,S.M. and Turchi,J.J. (1999) Replication Protein A (RPA) Binding to Duplex Cisplatin-Damaged DNA Is Mediated Through the Generation of Single-Stranded DNA.  J. Biol.	bind
22127	3	6716	5	13	NULL	NULL	NULL	single-stranded DNA	NucleicAcid	generation of	mediate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_23_4634_s_289	11095672	16       Patrick,S.M. and Turchi,J.J. (1999) Replication Protein A (RPA) Binding to Duplex Cisplatin-Damaged DNA Is Mediated Through the Generation of Single-Stranded DNA.  J. Biol.	bind
19190	1	6716	6	NULL	NULL	0	NULL	Replication Protein A	NULL		is	NULL				RPA	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_23_4634_s_289	11095672	16       Patrick,S.M. and Turchi,J.J. (1999) Replication Protein A (RPA) Binding to Duplex Cisplatin-Damaged DNA Is Mediated Through the Generation of Single-Stranded DNA.  J. Biol.	bind
19192	2	6716	6	NULL	NULL	0	NULL	RPA	NULL		bind	NULL				duplex DNA	NULL	Cisplatin-Damaged			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_23_4634_s_289	11095672	16       Patrick,S.M. and Turchi,J.J. (1999) Replication Protein A (RPA) Binding to Duplex Cisplatin-Damaged DNA Is Mediated Through the Generation of Single-Stranded DNA.  J. Biol.	bind
19193	3	6716	6	NULL	NULL	0	NULL	statement 2	NULL		is mediated through	NULL				single-stranded DNA	NULL	generation of			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_23_4634_s_289	11095672	16       Patrick,S.M. and Turchi,J.J. (1999) Replication Protein A (RPA) Binding to Duplex Cisplatin-Damaged DNA Is Mediated Through the Generation of Single-Stranded DNA.  J. Biol.	bind
22128	1	6717	5	13	NULL	NULL	NULL	U1A	GP		bind					RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_18_3841_s_262	11557816	16       Rimmele,M.E. and Belasco,J.G. (1998) Target discrimination by RNA-binding proteins: role of the ancillary protein U2A'' and a critical leucine residue in differentiating the RNA-binding specificity of spliceosomal proteins U1A and U2B'''.	bind
22129	2	6717	5	13	NULL	NULL	NULL	U2B	GP		bind					RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_18_3841_s_262	11557816	16       Rimmele,M.E. and Belasco,J.G. (1998) Target discrimination by RNA-binding proteins: role of the ancillary protein U2A'' and a critical leucine residue in differentiating the RNA-binding specificity of spliceosomal proteins U1A and U2B'''.	bind
44678	3	6717	5	13	NULL	NULL	NULL	U1A	GP		is a type of					spliceosomal protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_18_3841_s_262	11557816	16       Rimmele,M.E. and Belasco,J.G. (1998) Target discrimination by RNA-binding proteins: role of the ancillary protein U2A'' and a critical leucine residue in differentiating the RNA-binding specificity of spliceosomal proteins U1A and U2B'''.	bind
44679	4	6717	5	13	NULL	NULL	NULL	U2B	GP		is a type of					spliceosomal protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_18_3841_s_262	11557816	16       Rimmele,M.E. and Belasco,J.G. (1998) Target discrimination by RNA-binding proteins: role of the ancillary protein U2A'' and a critical leucine residue in differentiating the RNA-binding specificity of spliceosomal proteins U1A and U2B'''.	bind
56501	5	6717	5	13	NULL	NULL	NULL	U2A	GP		is a type of					ancillary protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_18_3841_s_262	11557816	16       Rimmele,M.E. and Belasco,J.G. (1998) Target discrimination by RNA-binding proteins: role of the ancillary protein U2A'' and a critical leucine residue in differentiating the RNA-binding specificity of spliceosomal proteins U1A and U2B'''.	bind
19194	1	6717	6	10	NULL	0	NULL	U1A			is a type of					spliceosomal protein					NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_18_3841_s_262	11557816	16       Rimmele,M.E. and Belasco,J.G. (1998) Target discrimination by RNA-binding proteins: role of the ancillary protein U2A'' and a critical leucine residue in differentiating the RNA-binding specificity of spliceosomal proteins U1A and U2B'''.	bind
19195	2	6717	6	10	NULL	0	NULL	U2B			is a type of					spliceosomal protein					NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_18_3841_s_262	11557816	16       Rimmele,M.E. and Belasco,J.G. (1998) Target discrimination by RNA-binding proteins: role of the ancillary protein U2A'' and a critical leucine residue in differentiating the RNA-binding specificity of spliceosomal proteins U1A and U2B'''.	bind
19199	3	6717	6	10	NULL	0	NULL	U2A			is a type of					ancillary protein					NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_18_3841_s_262	11557816	16       Rimmele,M.E. and Belasco,J.G. (1998) Target discrimination by RNA-binding proteins: role of the ancillary protein U2A'' and a critical leucine residue in differentiating the RNA-binding specificity of spliceosomal proteins U1A and U2B'''.	bind
44680	4	6717	6	10	NULL	0	NULL	U1A	NULL		bind	NULL				RNA	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_18_3841_s_262	11557816	16       Rimmele,M.E. and Belasco,J.G. (1998) Target discrimination by RNA-binding proteins: role of the ancillary protein U2A'' and a critical leucine residue in differentiating the RNA-binding specificity of spliceosomal proteins U1A and U2B'''.	bind
44682	5	6717	6	10	NULL	0	NULL	U2B	NULL		bind	NULL				RNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_18_3841_s_262	11557816	16       Rimmele,M.E. and Belasco,J.G. (1998) Target discrimination by RNA-binding proteins: role of the ancillary protein U2A'' and a critical leucine residue in differentiating the RNA-binding specificity of spliceosomal proteins U1A and U2B'''.	bind
22130	1	6718	5	13	NULL	NULL	NULL	DNA	NucleicAcid		bind		noncovalently			bis(1,10-phenanthroline)copper	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_24_4856_s_288	11121476	16       Veal,J.M., Merchant,K. and Rill,R.L. (1991) Noncovalent DNA binding of bis(1,10-phenanthroline)copper	bind
19201	1	6718	6	10	NULL	0	NULL	bis(1,10-phenanthroline)copper			bind		noncovalently			DNA					NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_24_4856_s_288	11121476	16       Veal,J.M., Merchant,K. and Rill,R.L. (1991) Noncovalent DNA binding of bis(1,10-phenanthroline)copper	bind
22131	1	6719	5	13	NULL	NULL	NULL	Lp(a)	GP		bind					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_129_s_25	8548413	16  17  Because it is an apoB-100 - containing particle, Lp(a) binds to the LDL receptor.	bind
44683	2	6719	5	13	NULL	NULL	NULL	Lp(a)	GP		contains					apoB-100	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_129_s_25	8548413	16  17  Because it is an apoB-100 - containing particle, Lp(a) binds to the LDL receptor.	bind
19202	1	6719	6	NULL	NULL	0	NULL	Lp(a)	NULL		bind	NULL				LDL receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_129_s_25	8548413	16  17  Because it is an apoB-100 - containing particle, Lp(a) binds to the LDL receptor.	bind
56503	2	6719	6	10	NULL	0	NULL	Lp(a)			contains					apoB-100					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_129_s_25	8548413	16  17  Because it is an apoB-100 - containing particle, Lp(a) binds to the LDL receptor.	bind
22132	1	6720	5	13	NULL	NULL	NULL	GP IIb/IIIa antagonists	Chemical	most	bind					GP IIb/IIa	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_4_437_s_33	10421606	16  Because most GP IIb/IIIa antagonists bind to GP IIb/IIa, irrespective of its state of activation, these antagonists inhibit the GP IIb/IIa receptor functions on unstimulated platelets.	bind
22133	2	6720	5	13	NULL	NULL	NULL	GP IIb/IIIa antagonists	Chemical		inhibit					GP IIb/IIa receptor	GP	function of			NULL	on unstimulated platelets	NULL	NULL	NULL	NULL	gw60_circulation_100_4_437_s_33	10421606	16  Because most GP IIb/IIIa antagonists bind to GP IIb/IIa, irrespective of its state of activation, these antagonists inhibit the GP IIb/IIa receptor functions on unstimulated platelets.	bind
56505	3	6720	5	13	NULL	NULL	NULL	statement 1	Process		occurs irrespective of					activation state	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_4_437_s_33	10421606	16  Because most GP IIb/IIIa antagonists bind to GP IIb/IIa, irrespective of its state of activation, these antagonists inhibit the GP IIb/IIa receptor functions on unstimulated platelets.	bind
19203	1	6720	6	NULL	NULL	0	NULL	GP IIb/IIIa antagonists	NULL		bind	NULL				GP IIb/IIa	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_100_4_437_s_33	10421606	16  Because most GP IIb/IIIa antagonists bind to GP IIb/IIa, irrespective of its state of activation, these antagonists inhibit the GP IIb/IIa receptor functions on unstimulated platelets.	bind
19204	2	6720	6	10	NULL	0	NULL	statement 1			occurs irrespective of					 activation state					NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_4_437_s_33	10421606	16  Because most GP IIb/IIIa antagonists bind to GP IIb/IIa, irrespective of its state of activation, these antagonists inhibit the GP IIb/IIa receptor functions on unstimulated platelets.	bind
19206	3	6720	6	10	NULL	0	NULL	GP IIb/IIIa antagonists			inhibit					GP IIb/IIa receptor		function of			NULL	unstimulated platelets	NULL	NULL	NULL	NULL	gw60_circulation_100_4_437_s_33	10421606	16  Because most GP IIb/IIIa antagonists bind to GP IIb/IIa, irrespective of its state of activation, these antagonists inhibit the GP IIb/IIa receptor functions on unstimulated platelets.	bind
22134	1	6721	5	13	NULL	NULL	NULL	GATA-3	GP		is a type of					GATA family of transcription factors	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_6_1945_s_140	12057898	16  GATA-3 belongs to the GATA family of transcription factors, which bind to the consensus sequence (A/T)GATA(A/G) and to the related motifs CGATGG and (T/A)GAT(T/A)(A/G).	bind
22135	2	6721	5	13	NULL	NULL	NULL	GATA-3	GP		bind							consensus sequence		(A/T)GATA(A/G)	NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_6_1945_s_140	12057898	16  GATA-3 belongs to the GATA family of transcription factors, which bind to the consensus sequence (A/T)GATA(A/G) and to the related motifs CGATGG and (T/A)GAT(T/A)(A/G).	bind
22136	3	6721	5	13	NULL	NULL	NULL	GATA-3	GP		bind									CGATGG	NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_6_1945_s_140	12057898	16  GATA-3 belongs to the GATA family of transcription factors, which bind to the consensus sequence (A/T)GATA(A/G) and to the related motifs CGATGG and (T/A)GAT(T/A)(A/G).	bind
22137	4	6721	5	13	NULL	NULL	NULL	GATA-3	GP		bind									(T/A)GAT(T/A)(A/G)	NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_6_1945_s_140	12057898	16  GATA-3 belongs to the GATA family of transcription factors, which bind to the consensus sequence (A/T)GATA(A/G) and to the related motifs CGATGG and (T/A)GAT(T/A)(A/G).	bind
19208	1	6721	6	10	NULL	0	NULL	GATA-3	NULL		is a type of	NULL				GATA family of transcription factors	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_6_1945_s_140	12057898	16  GATA-3 belongs to the GATA family of transcription factors, which bind to the consensus sequence (A/T)GATA(A/G) and to the related motifs CGATGG and (T/A)GAT(T/A)(A/G).	bind
19209	2	6721	6	10	NULL	0	NULL	GATA-3			bind							consensus sequence		(A/T)GATA(A/G)	NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_6_1945_s_140	12057898	16  GATA-3 belongs to the GATA family of transcription factors, which bind to the consensus sequence (A/T)GATA(A/G) and to the related motifs CGATGG and (T/A)GAT(T/A)(A/G).	bind
19211	3	6721	6	NULL	NULL	0	NULL	GATA-3	NULL		bind	NULL					NULL			CGATGG	NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_6_1945_s_140	12057898	16  GATA-3 belongs to the GATA family of transcription factors, which bind to the consensus sequence (A/T)GATA(A/G) and to the related motifs CGATGG and (T/A)GAT(T/A)(A/G).	bind
19212	4	6721	6	NULL	NULL	0	NULL	GATA-3	NULL		bind	NULL					NULL			(T/A)GAT(T/A)(A/G)	NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_6_1945_s_140	12057898	16  GATA-3 belongs to the GATA family of transcription factors, which bind to the consensus sequence (A/T)GATA(A/G) and to the related motifs CGATGG and (T/A)GAT(T/A)(A/G).	bind
22138	1	6722	5	13	NULL	NULL	NULL	PAI-1	GP		inhibit					cell migration	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_4_597_s_163	11157728	16  In addition, PAI-1 can inhibit cell migration by interfering with the binding of uPA receptor to vitronectin, independent of its function as a PAI. 39  These data suggest that alterations in the expression of PA system components may modulate intimal thickening via plasmin-dependent and plasmin-independent mechanisms.	bind
22139	2	6722	5	13	NULL	NULL	NULL	uPA receptor	GP		bind					vitronectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_4_597_s_163	11157728	16  In addition, PAI-1 can inhibit cell migration by interfering with the binding of uPA receptor to vitronectin, independent of its function as a PAI. 39  These data suggest that alterations in the expression of PA system components may modulate intimal thickening via plasmin-dependent and plasmin-independent mechanisms.	bind
22140	3	6722	5	13	NULL	NULL	NULL	PAI-1	GP		interferes with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_4_597_s_163	11157728	16  In addition, PAI-1 can inhibit cell migration by interfering with the binding of uPA receptor to vitronectin, independent of its function as a PAI. 39  These data suggest that alterations in the expression of PA system components may modulate intimal thickening via plasmin-dependent and plasmin-independent mechanisms.	bind
22141	4	6722	5	13	NULL	NULL	NULL	statement 3	Process		leads to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_4_597_s_163	11157728	16  In addition, PAI-1 can inhibit cell migration by interfering with the binding of uPA receptor to vitronectin, independent of its function as a PAI. 39  These data suggest that alterations in the expression of PA system components may modulate intimal thickening via plasmin-dependent and plasmin-independent mechanisms.	bind
22142	5	6722	5	13	NULL	NULL	NULL	statement 4	Process		is independent of					PAI	GP	function of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_4_597_s_163	11157728	16  In addition, PAI-1 can inhibit cell migration by interfering with the binding of uPA receptor to vitronectin, independent of its function as a PAI. 39  These data suggest that alterations in the expression of PA system components may modulate intimal thickening via plasmin-dependent and plasmin-independent mechanisms.	bind
22143	6	6722	5	13	NULL	NULL	NULL	PA system components	GP	alterations in the expression of	modulates					intimal thickening	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_4_597_s_163	11157728	16  In addition, PAI-1 can inhibit cell migration by interfering with the binding of uPA receptor to vitronectin, independent of its function as a PAI. 39  These data suggest that alterations in the expression of PA system components may modulate intimal thickening via plasmin-dependent and plasmin-independent mechanisms.	bind
22144	7	6722	5	13	NULL	NULL	NULL	statement 6	Process		via					plasmin-dependent mechanism	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_4_597_s_163	11157728	16  In addition, PAI-1 can inhibit cell migration by interfering with the binding of uPA receptor to vitronectin, independent of its function as a PAI. 39  These data suggest that alterations in the expression of PA system components may modulate intimal thickening via plasmin-dependent and plasmin-independent mechanisms.	bind
22145	8	6722	5	13	NULL	NULL	NULL	statement 6	Process		via					plasmin-independent mechanism	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_4_597_s_163	11157728	16  In addition, PAI-1 can inhibit cell migration by interfering with the binding of uPA receptor to vitronectin, independent of its function as a PAI. 39  These data suggest that alterations in the expression of PA system components may modulate intimal thickening via plasmin-dependent and plasmin-independent mechanisms.	bind
19213	1	6722	6	NULL	NULL	0	NULL	uPA receptor	NULL		bind	NULL				vitronectin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_4_597_s_163	11157728	16  In addition, PAI-1 can inhibit cell migration by interfering with the binding of uPA receptor to vitronectin, independent of its function as a PAI. 39  These data suggest that alterations in the expression of PA system components may modulate intimal thickening via plasmin-dependent and plasmin-independent mechanisms.	bind
19214	2	6722	6	NULL	NULL	0	NULL	PAI-1	NULL		inhibit	NULL				cell migration	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_4_597_s_163	11157728	16  In addition, PAI-1 can inhibit cell migration by interfering with the binding of uPA receptor to vitronectin, independent of its function as a PAI. 39  These data suggest that alterations in the expression of PA system components may modulate intimal thickening via plasmin-dependent and plasmin-independent mechanisms.	bind
19235	3	6722	6	NULL	NULL	0	NULL	statement 2	NULL		occurs via	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_4_597_s_163	11157728	16  In addition, PAI-1 can inhibit cell migration by interfering with the binding of uPA receptor to vitronectin, independent of its function as a PAI. 39  These data suggest that alterations in the expression of PA system components may modulate intimal thickening via plasmin-dependent and plasmin-independent mechanisms.	bind
19236	4	6722	6	NULL	NULL	0	NULL	PA system components	NULL	alterations in	modulate	NULL	may			intimal thickening	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_4_597_s_163	11157728	16  In addition, PAI-1 can inhibit cell migration by interfering with the binding of uPA receptor to vitronectin, independent of its function as a PAI. 39  These data suggest that alterations in the expression of PA system components may modulate intimal thickening via plasmin-dependent and plasmin-independent mechanisms.	bind
56519	5	6722	6	10	NULL	0	NULL	statement 3			is independent of					PAI		function of			NULL		0	NULL	NULL	NULL	gw60_circulation_103_4_597_s_163	11157728	16  In addition, PAI-1 can inhibit cell migration by interfering with the binding of uPA receptor to vitronectin, independent of its function as a PAI. 39  These data suggest that alterations in the expression of PA system components may modulate intimal thickening via plasmin-dependent and plasmin-independent mechanisms.	bind
56520	6	6722	6	10	NULL	0	NULL	statement 4			via					plasmin-dependent mechanism					NULL		0	NULL	NULL	NULL	gw60_circulation_103_4_597_s_163	11157728	16  In addition, PAI-1 can inhibit cell migration by interfering with the binding of uPA receptor to vitronectin, independent of its function as a PAI. 39  These data suggest that alterations in the expression of PA system components may modulate intimal thickening via plasmin-dependent and plasmin-independent mechanisms.	bind
56521	7	6722	6	10	NULL	0	NULL	statement 4			via					plasmin-independent mechanism					NULL		0	NULL	NULL	NULL	gw60_circulation_103_4_597_s_163	11157728	16  In addition, PAI-1 can inhibit cell migration by interfering with the binding of uPA receptor to vitronectin, independent of its function as a PAI. 39  These data suggest that alterations in the expression of PA system components may modulate intimal thickening via plasmin-dependent and plasmin-independent mechanisms.	bind
22146	1	6723	5	13	NULL	NULL	NULL	LPS	Chemical		bind					CD14	GP	soluble			NULL	 in serum	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_3_465_s_28	9102164	16  Recent evidence suggests that such activation occurs via LPS binding to soluble CD14 present in serum, with the resulting complex then binding to a cellular receptor.	bind
22147	2	6723	5	13	NULL	NULL	NULL	statement 1	Process		bind					cellular receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_3_465_s_28	9102164	16  Recent evidence suggests that such activation occurs via LPS binding to soluble CD14 present in serum, with the resulting complex then binding to a cellular receptor.	bind
22148	3	6723	5	13	NULL	NULL	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_3_465_s_28	9102164	16  Recent evidence suggests that such activation occurs via LPS binding to soluble CD14 present in serum, with the resulting complex then binding to a cellular receptor.	bind
19237	1	6723	6	10	NULL	0	NULL	LPS			bind					CD14		soluble			NULL	serum	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_3_465_s_28	9102164	16  Recent evidence suggests that such activation occurs via LPS binding to soluble CD14 present in serum, with the resulting complex then binding to a cellular receptor.	bind
56522	2	6723	6	10	NULL	0	NULL	statement 1			bind					cellular receptor					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_3_465_s_28	9102164	16  Recent evidence suggests that such activation occurs via LPS binding to soluble CD14 present in serum, with the resulting complex then binding to a cellular receptor.	bind
56523	3	6723	6	10	NULL	0	NULL	statement 1			leads to					statement 2					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_3_465_s_28	9102164	16  Recent evidence suggests that such activation occurs via LPS binding to soluble CD14 present in serum, with the resulting complex then binding to a cellular receptor.	bind
22149	1	6724	5	13	NULL	NULL	NULL	HL-60 cells	Cell		bind					platelet monolayers	Cell	thrombin-activated;;mouse			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_11_1124_s_42	9831707	16  RMP-1 inhibits binding of HL-60 cells to thrombin-activated mouse platelet monolayers and recombinant murine P-selectin.	bind
22150	2	6724	5	13	NULL	NULL	NULL	RMP-1	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_11_1124_s_42	9831707	16  RMP-1 inhibits binding of HL-60 cells to thrombin-activated mouse platelet monolayers and recombinant murine P-selectin.	bind
22151	3	6724	5	13	NULL	NULL	NULL	HL-60 cells	Cell		bind					P-selectin	GP	recombinant;;murine			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_11_1124_s_42	9831707	16  RMP-1 inhibits binding of HL-60 cells to thrombin-activated mouse platelet monolayers and recombinant murine P-selectin.	bind
22152	4	6724	5	13	NULL	NULL	NULL	RMP-1	GP		inhibit					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_11_1124_s_42	9831707	16  RMP-1 inhibits binding of HL-60 cells to thrombin-activated mouse platelet monolayers and recombinant murine P-selectin.	bind
19238	1	6724	6	10	NULL	0	NULL	HL-60 cells			bind					platelet monolayers		thrombin activated;;mouse			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_11_1124_s_42	9831707	16  RMP-1 inhibits binding of HL-60 cells to thrombin-activated mouse platelet monolayers and recombinant murine P-selectin.	bind
19239	2	6724	6	10	NULL	0	NULL	HL-60 cells			bind					P-selectin		recombinant;;murine			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_11_1124_s_42	9831707	16  RMP-1 inhibits binding of HL-60 cells to thrombin-activated mouse platelet monolayers and recombinant murine P-selectin.	bind
19240	3	6724	6	NULL	NULL	0	NULL	RMP-1	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_11_1124_s_42	9831707	16  RMP-1 inhibits binding of HL-60 cells to thrombin-activated mouse platelet monolayers and recombinant murine P-selectin.	bind
19241	4	6724	6	NULL	NULL	0	NULL	RMP-1	NULL		inhibits	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_11_1124_s_42	9831707	16  RMP-1 inhibits binding of HL-60 cells to thrombin-activated mouse platelet monolayers and recombinant murine P-selectin.	bind
22153	1	6725	5	13	NULL	NULL	NULL	TGF-betaR1	GP		is a type of					cell surface type I receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_109_s_22	11438459	16  TGF-beta1 signaling is transduced via cell surface type I and type II receptors (TGF-betaR1 and TGF-betaR2): TGF-betaR2 binds the ligand and forms a complex with TGF-betaR1 that activates intracellular signaling cascades.	bind
22154	2	6725	5	13	NULL	NULL	NULL	TGF-betaR2	GP		is a type of					cell surface type II receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_109_s_22	11438459	16  TGF-beta1 signaling is transduced via cell surface type I and type II receptors (TGF-betaR1 and TGF-betaR2): TGF-betaR2 binds the ligand and forms a complex with TGF-betaR1 that activates intracellular signaling cascades.	bind
22155	3	6725	5	13	NULL	NULL	NULL	TGF-beta1	Process	signalling	is transduced via					TGF-betaR1	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_109_s_22	11438459	16  TGF-beta1 signaling is transduced via cell surface type I and type II receptors (TGF-betaR1 and TGF-betaR2): TGF-betaR2 binds the ligand and forms a complex with TGF-betaR1 that activates intracellular signaling cascades.	bind
22156	4	6725	5	13	NULL	NULL	NULL	TGF-beta1	Process	signalling	is transduced via					TGF-betaR2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_109_s_22	11438459	16  TGF-beta1 signaling is transduced via cell surface type I and type II receptors (TGF-betaR1 and TGF-betaR2): TGF-betaR2 binds the ligand and forms a complex with TGF-betaR1 that activates intracellular signaling cascades.	bind
22157	5	6725	5	13	NULL	NULL	NULL	TGF-betaR2	GP		bind					ligand	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_109_s_22	11438459	16  TGF-beta1 signaling is transduced via cell surface type I and type II receptors (TGF-betaR1 and TGF-betaR2): TGF-betaR2 binds the ligand and forms a complex with TGF-betaR1 that activates intracellular signaling cascades.	bind
22158	6	6725	5	13	NULL	NULL	NULL	TGF-betaR2	GP		forms a complex with					TGF-betaR1	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_109_s_22	11438459	16  TGF-beta1 signaling is transduced via cell surface type I and type II receptors (TGF-betaR1 and TGF-betaR2): TGF-betaR2 binds the ligand and forms a complex with TGF-betaR1 that activates intracellular signaling cascades.	bind
22159	7	6725	5	13	NULL	NULL	NULL	TGF-betaR1	GP		activates					intracellular signaling cascades	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_109_s_22	11438459	16  TGF-beta1 signaling is transduced via cell surface type I and type II receptors (TGF-betaR1 and TGF-betaR2): TGF-betaR2 binds the ligand and forms a complex with TGF-betaR1 that activates intracellular signaling cascades.	bind
19466	1	6725	6	10	NULL	0	NULL	TGF-betaR1			transduces					TGF-beta1 		signaling of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_109_s_22	11438459	16  TGF-beta1 signaling is transduced via cell surface type I and type II receptors (TGF-betaR1 and TGF-betaR2): TGF-betaR2 binds the ligand and forms a complex with TGF-betaR1 that activates intracellular signaling cascades.	bind
19467	2	6725	6	10	NULL	0	NULL	TGF-betaR2			transduces					TGF-beta1 		signaling of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_109_s_22	11438459	16  TGF-beta1 signaling is transduced via cell surface type I and type II receptors (TGF-betaR1 and TGF-betaR2): TGF-betaR2 binds the ligand and forms a complex with TGF-betaR1 that activates intracellular signaling cascades.	bind
19468	3	6725	6	NULL	NULL	0	NULL	TGF-betaR2	NULL		bind	NULL				ligand	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_1_109_s_22	11438459	16  TGF-beta1 signaling is transduced via cell surface type I and type II receptors (TGF-betaR1 and TGF-betaR2): TGF-betaR2 binds the ligand and forms a complex with TGF-betaR1 that activates intracellular signaling cascades.	bind
19469	4	6725	6	NULL	NULL	0	NULL	statement 3	NULL		forms a complex with	NULL				TGF-betaR1	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_1_109_s_22	11438459	16  TGF-beta1 signaling is transduced via cell surface type I and type II receptors (TGF-betaR1 and TGF-betaR2): TGF-betaR2 binds the ligand and forms a complex with TGF-betaR1 that activates intracellular signaling cascades.	bind
19470	5	6725	6	NULL	NULL	0	NULL	statement 4	NULL		activates	NULL				intracellular signaling cascades	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_1_109_s_22	11438459	16  TGF-beta1 signaling is transduced via cell surface type I and type II receptors (TGF-betaR1 and TGF-betaR2): TGF-betaR2 binds the ligand and forms a complex with TGF-betaR1 that activates intracellular signaling cascades.	bind
56524	6	6725	6	10	NULL	0	NULL	TGF-betaR1			is a type of					cell surface type I receptor					NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_1_109_s_22	11438459	16  TGF-beta1 signaling is transduced via cell surface type I and type II receptors (TGF-betaR1 and TGF-betaR2): TGF-betaR2 binds the ligand and forms a complex with TGF-betaR1 that activates intracellular signaling cascades.	bind
56525	7	6725	6	10	NULL	0	NULL	TGF-betaR2			is a type of					cell surface type II receptor					NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_1_109_s_22	11438459	16  TGF-beta1 signaling is transduced via cell surface type I and type II receptors (TGF-betaR1 and TGF-betaR2): TGF-betaR2 binds the ligand and forms a complex with TGF-betaR1 that activates intracellular signaling cascades.	bind
22241	1	6726	5	13	NULL	NULL	NULL	heparin	Chemical		bind		non-specifically			plasma proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_1_118_s_33	8994426	16  These observations may explain why the anticoagulant response, as measured by anti-Xa levels, is more predictable for LMWH than for UFH. 14  We also demonstrated that the extent of nonspecific binding of heparin to plasma proteins is dependent on the molecular weight of the heparin chains, with the longer chains exhibiting the most nonspecific binding.	bind
22242	3	6726	5	13	NULL	NULL	NULL	statement 2	Process		is greater than					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_1_118_s_33	8994426	16  These observations may explain why the anticoagulant response, as measured by anti-Xa levels, is more predictable for LMWH than for UFH. 14  We also demonstrated that the extent of nonspecific binding of heparin to plasma proteins is dependent on the molecular weight of the heparin chains, with the longer chains exhibiting the most nonspecific binding.	bind
22243	2	6726	5	13	NULL	NULL	NULL	heparin	Chemical	longer chains of	bind		non-specifically			plasma proteins	GP	 			NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_1_118_s_33	8994426	16  These observations may explain why the anticoagulant response, as measured by anti-Xa levels, is more predictable for LMWH than for UFH. 14  We also demonstrated that the extent of nonspecific binding of heparin to plasma proteins is dependent on the molecular weight of the heparin chains, with the longer chains exhibiting the most nonspecific binding.	bind
58590	4	6726	5	13	NULL	NULL	NULL	statement 1	Process		depends on					heparin	Chemical	molecular weight of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_1_118_s_33	8994426	16  These observations may explain why the anticoagulant response, as measured by anti-Xa levels, is more predictable for LMWH than for UFH. 14  We also demonstrated that the extent of nonspecific binding of heparin to plasma proteins is dependent on the molecular weight of the heparin chains, with the longer chains exhibiting the most nonspecific binding.	bind
19242	1	6726	6	NULL	NULL	0	NULL	heparin	NULL		bind	NULL	non-specifically			plasma proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_95_1_118_s_33	8994426	16  These observations may explain why the anticoagulant response, as measured by anti-Xa levels, is more predictable for LMWH than for UFH. 14  We also demonstrated that the extent of nonspecific binding of heparin to plasma proteins is dependent on the molecular weight of the heparin chains, with the longer chains exhibiting the most nonspecific binding.	bind
19243	4	6726	6	10	NULL	0	NULL	statement 1			is dependent on					heparin chains		molecular weight of 			NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_1_118_s_33	8994426	16  These observations may explain why the anticoagulant response, as measured by anti-Xa levels, is more predictable for LMWH than for UFH. 14  We also demonstrated that the extent of nonspecific binding of heparin to plasma proteins is dependent on the molecular weight of the heparin chains, with the longer chains exhibiting the most nonspecific binding.	bind
56526	2	6726	6	10	NULL	0	NULL	heparin		longer chains of	bind		non-specifically			plasma proteins					NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_1_118_s_33	8994426	16  These observations may explain why the anticoagulant response, as measured by anti-Xa levels, is more predictable for LMWH than for UFH. 14  We also demonstrated that the extent of nonspecific binding of heparin to plasma proteins is dependent on the molecular weight of the heparin chains, with the longer chains exhibiting the most nonspecific binding.	bind
58591	3	6726	6	10	NULL	0	NULL	statement 2			is greater than					statement 1					NULL		0	NULL	NULL	NULL	gw60_circulation_95_1_118_s_33	8994426	16  These observations may explain why the anticoagulant response, as measured by anti-Xa levels, is more predictable for LMWH than for UFH. 14  We also demonstrated that the extent of nonspecific binding of heparin to plasma proteins is dependent on the molecular weight of the heparin chains, with the longer chains exhibiting the most nonspecific binding.	bind
22244	1	6727	5	13	NULL	NULL	NULL	TFPI	GP	 125I-labeled;; heparin-releasable	bind					LDL/VLDL	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_879_s_183	7600119	16  This hypothesis has been supported by animal studies by Novotny et al, 12  who demonstrated that exogenously added 125I-labeled heparin-releasable TFPI can bind LDL/VLDL and HDL in vivo.	bind
22246	2	6727	5	13	NULL	NULL	NULL	TFPI	GP	 125I-labeled;; heparin-releasable	bind					HDL	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_879_s_183	7600119	16  This hypothesis has been supported by animal studies by Novotny et al, 12  who demonstrated that exogenously added 125I-labeled heparin-releasable TFPI can bind LDL/VLDL and HDL in vivo.	bind
19244	1	6727	6	10	NULL	0	NULL	TFPI	NULL	125I-labeled;;heparin-releasable	bind	NULL				LDL/VLDL	NULL				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_879_s_183	7600119	16  This hypothesis has been supported by animal studies by Novotny et al, 12  who demonstrated that exogenously added 125I-labeled heparin-releasable TFPI can bind LDL/VLDL and HDL in vivo.	bind
19245	2	6727	6	10	NULL	0	NULL	TFPI	NULL	125I-labeled;; heparin-releasable	bind	NULL				HDL	NULL				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_879_s_183	7600119	16  This hypothesis has been supported by animal studies by Novotny et al, 12  who demonstrated that exogenously added 125I-labeled heparin-releasable TFPI can bind LDL/VLDL and HDL in vivo.	bind
22251	1	6728	5	13	NULL	NULL	NULL	FXa	GP		bind								second Kunitz-type domain		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_11_2055_s_24	7583589	16  Thus, binding of FXa by the second Kunitz-type domain potentiates inhibition of the TF-FVIIa complex by the first Kunitz-type domain.	bind
22252	2	6728	5	13	NULL	NULL	NULL				inhibit			first Kunitz-type domain		TF-FVIIa complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_11_2055_s_24	7583589	16  Thus, binding of FXa by the second Kunitz-type domain potentiates inhibition of the TF-FVIIa complex by the first Kunitz-type domain.	bind
22253	3	6728	5	13	NULL	NULL	NULL	statement 1	Process		potentiate					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_11_2055_s_24	7583589	16  Thus, binding of FXa by the second Kunitz-type domain potentiates inhibition of the TF-FVIIa complex by the first Kunitz-type domain.	bind
19246	1	6728	6	NULL	NULL	0	NULL	FXa	NULL		bind	NULL					NULL		Kunitz-type domain		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_11_2055_s_24	7583589	16  Thus, binding of FXa by the second Kunitz-type domain potentiates inhibition of the TF-FVIIa complex by the first Kunitz-type domain.	bind
19471	2	6728	6	NULL	NULL	0	NULL	statement 1	NULL		potentiates	NULL				TF-FVIIa complex	NULL	inhibition of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_11_2055_s_24	7583589	16  Thus, binding of FXa by the second Kunitz-type domain potentiates inhibition of the TF-FVIIa complex by the first Kunitz-type domain.	bind
19472	3	6728	6	NULL	NULL	0	NULL	statement 2	NULL		occurs via	NULL					NULL	first	Kunitz-type domain		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_11_2055_s_24	7583589	16  Thus, binding of FXa by the second Kunitz-type domain potentiates inhibition of the TF-FVIIa complex by the first Kunitz-type domain.	bind
22255	1	6729	5	13	NULL	NULL	NULL	MBL	GP		bind		may			CK1	GP		head region		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_1045_s_267	11549596	16  Thus, MBL may bind the CK1 head and/or tail region(s) after endothelial oxidative stress.	bind
22256	2	6729	5	13	NULL	NULL	NULL	MBL	GP		bind		may			CK1	GP		tail region		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_1045_s_267	11549596	16  Thus, MBL may bind the CK1 head and/or tail region(s) after endothelial oxidative stress.	bind
22257	3	6729	5	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_1045_s_267	11549596	16  Thus, MBL may bind the CK1 head and/or tail region(s) after endothelial oxidative stress.	bind
22258	4	6729	5	13	NULL	NULL	NULL	statement 1	Process		occurs after					oxidative stress	Process	endothelial			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_1045_s_267	11549596	16  Thus, MBL may bind the CK1 head and/or tail region(s) after endothelial oxidative stress.	bind
22260	5	6729	5	13	NULL	NULL	NULL	statement 2	Process		occurs after					oxidative stress	Process	endothelial			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_1045_s_267	11549596	16  Thus, MBL may bind the CK1 head and/or tail region(s) after endothelial oxidative stress.	bind
19247	1	6729	6	NULL	NULL	0	NULL	MBL	NULL		bind	NULL	may			CK1	NULL		head region		NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_3_1045_s_267	11549596	16  Thus, MBL may bind the CK1 head and/or tail region(s) after endothelial oxidative stress.	bind
19248	2	6729	6	NULL	NULL	0	NULL	MBL	NULL		bind	NULL	may			CK1	NULL		tail region		NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_3_1045_s_267	11549596	16  Thus, MBL may bind the CK1 head and/or tail region(s) after endothelial oxidative stress.	bind
19249	3	6729	6	NULL	NULL	0	NULL	statement 1	NULL		occurs after	NULL				oxidative stress 	NULL	endothelial			NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_3_1045_s_267	11549596	16  Thus, MBL may bind the CK1 head and/or tail region(s) after endothelial oxidative stress.	bind
19250	4	6729	6	NULL	NULL	0	NULL	statement 2	NULL		occurs after	NULL				oxidative stress	NULL	endothelial			NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_3_1045_s_267	11549596	16  Thus, MBL may bind the CK1 head and/or tail region(s) after endothelial oxidative stress.	bind
19251	5	6729	6	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_3_1045_s_267	11549596	16  Thus, MBL may bind the CK1 head and/or tail region(s) after endothelial oxidative stress.	bind
22262	1	6730	5	13	NULL	NULL	NULL	Trx	GP	oxidized form	does not bind			intramolecular disulfide between C32 and C35		ASK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1259_s_33	12089063	16 -  18 The oxidized form (intramolecular disulfide between C32 and C35) or redox-inactive form (the double-mutation at catalytic sites C32 and C35) of Trx does not bind to ASK1.	bind
22263	2	6730	5	13	NULL	NULL	NULL	Trx	GP	redox-inactive form;;double-mutant	does not bind			catalytic sites C32 and C35		ASK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1259_s_33	12089063	16 -  18 The oxidized form (intramolecular disulfide between C32 and C35) or redox-inactive form (the double-mutation at catalytic sites C32 and C35) of Trx does not bind to ASK1.	bind
19252	1	6730	6	NULL	NULL	0	NULL	Trx	NULL	oxidized form	does not bind	NULL		intramolecular disulfide between C32 and C35		ASK1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_12_1259_s_33	12089063	16 -  18 The oxidized form (intramolecular disulfide between C32 and C35) or redox-inactive form (the double-mutation at catalytic sites C32 and C35) of Trx does not bind to ASK1.	bind
19253	2	6730	6	10	NULL	0	NULL	Trx		redox-inactive form;;double mutants	does not bind			catalytic sites C32 and C35		ASK1					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1259_s_33	12089063	16 -  18 The oxidized form (intramolecular disulfide between C32 and C35) or redox-inactive form (the double-mutation at catalytic sites C32 and C35) of Trx does not bind to ASK1.	bind
22265	1	6731	5	13	NULL	NULL	NULL	VWF	GP		bind					GPIb-IX-V	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2131_s_26	14500287	16 - 18   Here also VWF binds to its platelet membrane receptor, GPIb-IX-V, establishing a transient bond that slows down platelets and thus facilitates their activation.	bind
22267	3	6731	5	13	NULL	NULL	NULL	statement 1	Process		slows down					platelets	Cell				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2131_s_26	14500287	16 - 18   Here also VWF binds to its platelet membrane receptor, GPIb-IX-V, establishing a transient bond that slows down platelets and thus facilitates their activation.	bind
22268	4	6731	5	13	NULL	NULL	NULL	statement 3	Process		facilitates					platelets	Cell	activation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2131_s_26	14500287	16 - 18   Here also VWF binds to its platelet membrane receptor, GPIb-IX-V, establishing a transient bond that slows down platelets and thus facilitates their activation.	bind
56527	2	6731	5	13	NULL	NULL	NULL	GPIb-IX-V	GP		is a type of					platelet membrane receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2131_s_26	14500287	16 - 18   Here also VWF binds to its platelet membrane receptor, GPIb-IX-V, establishing a transient bond that slows down platelets and thus facilitates their activation.	bind
19254	1	6731	6	NULL	NULL	0	NULL	VWF	NULL		bind	NULL				GPIb-IX-V	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2131_s_26	14500287	16 - 18   Here also VWF binds to its platelet membrane receptor, GPIb-IX-V, establishing a transient bond that slows down platelets and thus facilitates their activation.	bind
19255	2	6731	6	10	NULL	0	NULL	GPIb-IX-V			is a type of					platelet membrane receptor					NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2131_s_26	14500287	16 - 18   Here also VWF binds to its platelet membrane receptor, GPIb-IX-V, establishing a transient bond that slows down platelets and thus facilitates their activation.	bind
19256	4	6731	6	10	NULL	0	NULL	statement 3			facilitate					platelets		activation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2131_s_26	14500287	16 - 18   Here also VWF binds to its platelet membrane receptor, GPIb-IX-V, establishing a transient bond that slows down platelets and thus facilitates their activation.	bind
19257	3	6731	6	10	NULL	0	NULL	statement 1			slows down					platelets					NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2131_s_26	14500287	16 - 18   Here also VWF binds to its platelet membrane receptor, GPIb-IX-V, establishing a transient bond that slows down platelets and thus facilitates their activation.	bind
22270	1	6732	5	13	NULL	NULL	NULL	apoB	GP		bind		covalently	cysteine residue		apo(a)	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2219_s_34	15345512	16 - 18   Notably, the cysteine residue in apoB involved in the covalent bond between apoB and apo(a) is close to the postulated LDL receptor-binding region of apoB.	bind
22278	2	6732	5	13	NULL	NULL	NULL	statement 1	Process		is close to					apoB	GP		LDL receptor-binding region		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2219_s_34	15345512	16 - 18   Notably, the cysteine residue in apoB involved in the covalent bond between apoB and apo(a) is close to the postulated LDL receptor-binding region of apoB.	bind
19335	1	6732	6	10	NULL	0	NULL	apoB			bind		covalently	cysteine residue		apo(a)					NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2219_s_34	15345512	16 - 18   Notably, the cysteine residue in apoB involved in the covalent bond between apoB and apo(a) is close to the postulated LDL receptor-binding region of apoB.	bind
56528	2	6732	6	10	NULL	0	NULL	statement 1			is close to					apoB			LDL receptor-binding region of 		NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2219_s_34	15345512	16 - 18   Notably, the cysteine residue in apoB involved in the covalent bond between apoB and apo(a) is close to the postulated LDL receptor-binding region of apoB.	bind
22279	1	6733	5	13	NULL	NULL	NULL	HB-EGF	GP	soluble	bind					HSPG	GP				NULL	on the surface of SMCs	NULL	NULL	NULL	NULL	gw70_circulation_108_21_2679_s_147	14623816	16 - 19    Because most of the soluble HB-EGF binds to HSPG on the surface of SMCs, 20 membrane-associated soluble HB-EGF reflects the amount of HB-EGF shedding.	bind
19336	1	6733	6	NULL	NULL	0	NULL	HB-EGF	NULL	soluble	bind	NULL				HSPG	NULL				NULL	surface of SMCs	0	NULL	NULL	NULL	gw70_circulation_108_21_2679_s_147	14623816	16 - 19    Because most of the soluble HB-EGF binds to HSPG on the surface of SMCs, 20 membrane-associated soluble HB-EGF reflects the amount of HB-EGF shedding.	bind
22281	1	6734	5	13	NULL	NULL	NULL	PI3-K	GP		bind			p85 regulatory subunit of		IRS-1 variant	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_109_3_399_s_127	14707024	16 - 20     Thus, it has been demonstrated that the presence of the Gly Arg change at codon 972-IRS-1 causes a specific defect in binding of the p85 regulatory subunit of PI3-K to the IRS-1 variant.	bind
22284	2	6734	5	13	NULL	NULL	NULL			change of	occurs at			Gly Arg		IRS-1	GP			codon 972	NULL		NULL	NULL	NULL	NULL	gw70_circulation_109_3_399_s_127	14707024	16 - 20     Thus, it has been demonstrated that the presence of the Gly Arg change at codon 972-IRS-1 causes a specific defect in binding of the p85 regulatory subunit of PI3-K to the IRS-1 variant.	bind
22285	3	6734	5	13	NULL	NULL	NULL	statement 2	Process		causes					statement 1	Process	specific defect in			NULL		NULL	NULL	NULL	NULL	gw70_circulation_109_3_399_s_127	14707024	16 - 20     Thus, it has been demonstrated that the presence of the Gly Arg change at codon 972-IRS-1 causes a specific defect in binding of the p85 regulatory subunit of PI3-K to the IRS-1 variant.	bind
19337	1	6734	6	NULL	NULL	0	NULL	PI3-K 	NULL		bind	NULL		p85 regulatory subunit		IRS-1 variant	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_109_3_399_s_127	14707024	16 - 20     Thus, it has been demonstrated that the presence of the Gly Arg change at codon 972-IRS-1 causes a specific defect in binding of the p85 regulatory subunit of PI3-K to the IRS-1 variant.	bind
19338	2	6734	6	NULL	NULL	0	NULL	IRS-1	NULL		causes	NULL		Gly Arg change at codon 972		statement 1	NULL	defect in 			NULL		0	NULL	NULL	NULL	gw70_circulation_109_3_399_s_127	14707024	16 - 20     Thus, it has been demonstrated that the presence of the Gly Arg change at codon 972-IRS-1 causes a specific defect in binding of the p85 regulatory subunit of PI3-K to the IRS-1 variant.	bind
22286	1	6736	5	13	NULL	NULL	NULL	ryanodine	Chemical		bind					SR release channel	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_12_1192_s_31	null	16 17  Furthermore, McCall et al 15  found that BayK increased binding of ryanodine to the SR release channel, but only under conditions in which sarcolemmal-SR junctions may be expected to be intact (ie, not after physical disruption).	bind
22287	2	6736	5	13	NULL	NULL	NULL	BayK	Chemical		increase					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_12_1192_s_31	null	16 17  Furthermore, McCall et al 15  found that BayK increased binding of ryanodine to the SR release channel, but only under conditions in which sarcolemmal-SR junctions may be expected to be intact (ie, not after physical disruption).	bind
22288	3	6736	5	13	NULL	NULL	NULL	statement 2	Process		occurs in		only			sarcolemmal-SR junctions	OrganismPart	intact			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_12_1192_s_31	null	16 17  Furthermore, McCall et al 15  found that BayK increased binding of ryanodine to the SR release channel, but only under conditions in which sarcolemmal-SR junctions may be expected to be intact (ie, not after physical disruption).	bind
19340	1	6736	6	NULL	NULL	0	NULL	ryanodine	NULL		bind	NULL				SR release channel	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_12_1192_s_31	null	16 17  Furthermore, McCall et al 15  found that BayK increased binding of ryanodine to the SR release channel, but only under conditions in which sarcolemmal-SR junctions may be expected to be intact (ie, not after physical disruption).	bind
19341	2	6736	6	NULL	NULL	0	NULL	BayK	NULL		increases	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_12_1192_s_31	null	16 17  Furthermore, McCall et al 15  found that BayK increased binding of ryanodine to the SR release channel, but only under conditions in which sarcolemmal-SR junctions may be expected to be intact (ie, not after physical disruption).	bind
19342	3	6736	6	NULL	NULL	0	NULL	statement 2	NULL		occurs in presence of	NULL	only			intact sarcolemmal-SR junctions	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_12_1192_s_31	null	16 17  Furthermore, McCall et al 15  found that BayK increased binding of ryanodine to the SR release channel, but only under conditions in which sarcolemmal-SR junctions may be expected to be intact (ie, not after physical disruption).	bind
22295	1	6737	5	13	NULL	NULL	NULL	heparan sulfate	Chemical		is required for					FGF-2 receptor	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_9_981_s_173	10468530	16 17  In addition, heparin can substitute for heparan sulfate as a required factor for FGF-2 receptor binding and may separately bind FGF to cells and facilitate internalization.	bind
22297	2	6737	5	13	NULL	NULL	NULL	heparin	Chemical		is required for					FGF-2 receptor	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_9_981_s_173	10468530	16 17  In addition, heparin can substitute for heparan sulfate as a required factor for FGF-2 receptor binding and may separately bind FGF to cells and facilitate internalization.	bind
22298	3	6737	5	13	NULL	NULL	NULL	statement 2	Process		substitutes for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_9_981_s_173	10468530	16 17  In addition, heparin can substitute for heparan sulfate as a required factor for FGF-2 receptor binding and may separately bind FGF to cells and facilitate internalization.	bind
22300	4	6737	5	13	NULL	NULL	NULL	FGF	GP		binds to					cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_9_981_s_173	10468530	16 17  In addition, heparin can substitute for heparan sulfate as a required factor for FGF-2 receptor binding and may separately bind FGF to cells and facilitate internalization.	bind
22302	6	6737	5	13	NULL	NULL	NULL	statement 5	Process		facilitates					internalization	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_9_981_s_173	10468530	16 17  In addition, heparin can substitute for heparan sulfate as a required factor for FGF-2 receptor binding and may separately bind FGF to cells and facilitate internalization.	bind
44684	5	6737	5	13	NULL	NULL	NULL	heparin	Chemical		bind		may;;separately			statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_9_981_s_173	10468530	16 17  In addition, heparin can substitute for heparan sulfate as a required factor for FGF-2 receptor binding and may separately bind FGF to cells and facilitate internalization.	bind
19473	1	6737	6	NULL	NULL	0	NULL	heparan sulfate	NULL		is required for	NULL				FGF-2 receptor	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_circulation_100_9_981_s_173	10468530	16 17  In addition, heparin can substitute for heparan sulfate as a required factor for FGF-2 receptor binding and may separately bind FGF to cells and facilitate internalization.	bind
19475	2	6737	6	10	NULL	0	NULL	FGF			bind		may			cells					NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_9_981_s_173	10468530	16 17  In addition, heparin can substitute for heparan sulfate as a required factor for FGF-2 receptor binding and may separately bind FGF to cells and facilitate internalization.	bind
19476	3	6737	6	10	NULL	0	NULL	heparin			bind		may;;separately			statement 2					NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_9_981_s_173	10468530	16 17  In addition, heparin can substitute for heparan sulfate as a required factor for FGF-2 receptor binding and may separately bind FGF to cells and facilitate internalization.	bind
56529	4	6737	6	10	NULL	0	NULL	heparin			is required for					FGF-2 receptor		binding of			NULL		0	NULL	NULL	NULL	gw60_circulation_100_9_981_s_173	10468530	16 17  In addition, heparin can substitute for heparan sulfate as a required factor for FGF-2 receptor binding and may separately bind FGF to cells and facilitate internalization.	bind
56530	5	6737	6	10	NULL	0	NULL	statement 2			substitutes for					statement 1					NULL		0	NULL	NULL	NULL	gw60_circulation_100_9_981_s_173	10468530	16 17  In addition, heparin can substitute for heparan sulfate as a required factor for FGF-2 receptor binding and may separately bind FGF to cells and facilitate internalization.	bind
56531	6	6737	6	10	NULL	0	NULL	statement 3			facilitate					internalization					NULL		0	NULL	NULL	NULL	gw60_circulation_100_9_981_s_173	10468530	16 17  In addition, heparin can substitute for heparan sulfate as a required factor for FGF-2 receptor binding and may separately bind FGF to cells and facilitate internalization.	bind
22301	1	6738	5	13	NULL	NULL	NULL	vWF	GP		bind					GPIb	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_64_s_34	8548428	16 17  There is evidence that the binding of vWF to GPIb induced by botrocetin is localized elsewhere within the disulfide-bonded loop.	bind
22303	2	6738	5	13	NULL	NULL	NULL	botrocetin	Chemical		induces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_64_s_34	8548428	16 17  There is evidence that the binding of vWF to GPIb induced by botrocetin is localized elsewhere within the disulfide-bonded loop.	bind
22305	3	6738	5	13	NULL	NULL	NULL	statement 2	Process		is localized within					disulfide-bonded loop	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_64_s_34	8548428	16 17  There is evidence that the binding of vWF to GPIb induced by botrocetin is localized elsewhere within the disulfide-bonded loop.	bind
19343	1	6738	6	NULL	NULL	0	NULL	vWF	NULL		bind	NULL				GPIb	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_64_s_34	8548428	16 17  There is evidence that the binding of vWF to GPIb induced by botrocetin is localized elsewhere within the disulfide-bonded loop.	bind
19344	2	6738	6	NULL	NULL	0	NULL	botrocetin	NULL		induces	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_64_s_34	8548428	16 17  There is evidence that the binding of vWF to GPIb induced by botrocetin is localized elsewhere within the disulfide-bonded loop.	bind
56532	3	6738	6	10	NULL	0	NULL	statement 2			is localized within					disulfide-bonded loop					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_64_s_34	8548428	16 17  There is evidence that the binding of vWF to GPIb induced by botrocetin is localized elsewhere within the disulfide-bonded loop.	bind
22306	1	6739	5	13	NULL	NULL	NULL	VEGF-C	GP		bind					VEGFR-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_11_992_s_25	10571529	16 17  VEGF-C and VEGF-D bind both VEGFR-2 and VEGFR-3/Flt4 and constitute a subgroup within the VEGF family characterized by N- and C-terminal extensions flanking the VEGF homology domain.	bind
22307	2	6739	5	13	NULL	NULL	NULL	VEGF-C	GP		bind					VEGFR-3/Flt4	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_11_992_s_25	10571529	16 17  VEGF-C and VEGF-D bind both VEGFR-2 and VEGFR-3/Flt4 and constitute a subgroup within the VEGF family characterized by N- and C-terminal extensions flanking the VEGF homology domain.	bind
22308	3	6739	5	13	NULL	NULL	NULL	VEGF-D	GP		bind					VEGFR-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_11_992_s_25	10571529	16 17  VEGF-C and VEGF-D bind both VEGFR-2 and VEGFR-3/Flt4 and constitute a subgroup within the VEGF family characterized by N- and C-terminal extensions flanking the VEGF homology domain.	bind
22309	4	6739	5	13	NULL	NULL	NULL	VEGF-D	GP		bind					VEGFR-3/Flt4	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_11_992_s_25	10571529	16 17  VEGF-C and VEGF-D bind both VEGFR-2 and VEGFR-3/Flt4 and constitute a subgroup within the VEGF family characterized by N- and C-terminal extensions flanking the VEGF homology domain.	bind
22310	5	6739	5	13	NULL	NULL	NULL	VEGF-C	GP		constitutes					VEGF family	GP	a subgroup within			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_11_992_s_25	10571529	16 17  VEGF-C and VEGF-D bind both VEGFR-2 and VEGFR-3/Flt4 and constitute a subgroup within the VEGF family characterized by N- and C-terminal extensions flanking the VEGF homology domain.	bind
22311	6	6739	5	13	NULL	NULL	NULL	VEGF-D	GP		constitutes					VEGF family	GP	a subgroup within			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_11_992_s_25	10571529	16 17  VEGF-C and VEGF-D bind both VEGFR-2 and VEGFR-3/Flt4 and constitute a subgroup within the VEGF family characterized by N- and C-terminal extensions flanking the VEGF homology domain.	bind
22313	7	6739	5	13	NULL	NULL	NULL	statement 5	GP		is characterized by								N-terminal extension flanking VEGF homology domain		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_11_992_s_25	10571529	16 17  VEGF-C and VEGF-D bind both VEGFR-2 and VEGFR-3/Flt4 and constitute a subgroup within the VEGF family characterized by N- and C-terminal extensions flanking the VEGF homology domain.	bind
22314	8	6739	5	13	NULL	NULL	NULL	statement 6	GP		is characterized by								C-terminal extension flanking VEGF homology domain		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_11_992_s_25	10571529	16 17  VEGF-C and VEGF-D bind both VEGFR-2 and VEGFR-3/Flt4 and constitute a subgroup within the VEGF family characterized by N- and C-terminal extensions flanking the VEGF homology domain.	bind
19345	1	6739	6	10	NULL	0	NULL	VEGF-C			bind					VEGFR-2					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_11_992_s_25	10571529	16 17  VEGF-C and VEGF-D bind both VEGFR-2 and VEGFR-3/Flt4 and constitute a subgroup within the VEGF family characterized by N- and C-terminal extensions flanking the VEGF homology domain.	bind
19346	2	6739	6	NULL	NULL	0	NULL	VEGF-C	NULL		bind	NULL				VEGFR-3/Flt4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_85_11_992_s_25	10571529	16 17  VEGF-C and VEGF-D bind both VEGFR-2 and VEGFR-3/Flt4 and constitute a subgroup within the VEGF family characterized by N- and C-terminal extensions flanking the VEGF homology domain.	bind
19347	3	6739	6	NULL	NULL	0	NULL	VEGF-D	NULL		bind	NULL				VEGFR-2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_85_11_992_s_25	10571529	16 17  VEGF-C and VEGF-D bind both VEGFR-2 and VEGFR-3/Flt4 and constitute a subgroup within the VEGF family characterized by N- and C-terminal extensions flanking the VEGF homology domain.	bind
19348	4	6739	6	NULL	NULL	0	NULL	VEGF-D	NULL		bind	NULL				VEGFR-3/Flt4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_85_11_992_s_25	10571529	16 17  VEGF-C and VEGF-D bind both VEGFR-2 and VEGFR-3/Flt4 and constitute a subgroup within the VEGF family characterized by N- and C-terminal extensions flanking the VEGF homology domain.	bind
56533	5	6739	6	10	NULL	0	NULL	VEGF-C			constitute					VEGF family		a subgroup within			NULL		0	NULL	NULL	NULL	gw60_circulationres_85_11_992_s_25	10571529	16 17  VEGF-C and VEGF-D bind both VEGFR-2 and VEGFR-3/Flt4 and constitute a subgroup within the VEGF family characterized by N- and C-terminal extensions flanking the VEGF homology domain.	bind
56534	6	6739	6	10	NULL	0	NULL	VEGF-D			constitute					VEGF family		a subgroup within			NULL		0	NULL	NULL	NULL	gw60_circulationres_85_11_992_s_25	10571529	16 17  VEGF-C and VEGF-D bind both VEGFR-2 and VEGFR-3/Flt4 and constitute a subgroup within the VEGF family characterized by N- and C-terminal extensions flanking the VEGF homology domain.	bind
56535	7	6739	6	10	NULL	0	NULL	statement 5			characterized by								N-terminal extension flanking the VEGF homology domain		NULL		0	NULL	NULL	NULL	gw60_circulationres_85_11_992_s_25	10571529	16 17  VEGF-C and VEGF-D bind both VEGFR-2 and VEGFR-3/Flt4 and constitute a subgroup within the VEGF family characterized by N- and C-terminal extensions flanking the VEGF homology domain.	bind
56536	8	6739	6	10	NULL	0	NULL	statement 6			characterized by								C-terminal extension flanking the VEGF homology domain		NULL		0	NULL	NULL	NULL	gw60_circulationres_85_11_992_s_25	10571529	16 17  VEGF-C and VEGF-D bind both VEGFR-2 and VEGFR-3/Flt4 and constitute a subgroup within the VEGF family characterized by N- and C-terminal extensions flanking the VEGF homology domain.	bind
24818	1	6741	5	13	NULL	NULL	NULL	receptor-associated kinases	GP	of JAK family	bind					AT1 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_6_1053_s_188	7586216	16 17 38 39  The fact that the receptor-associated kinases of the JAK family bind to the AT1 receptor and phosphorylate the STAT family of transcription factors 36  suggests that the long-term effects of Ang II on gene expression may resemble those of tyrosine kinase - coupled receptors, such as the PDGF receptor, and classic cytokine receptors, such as the interleukin and interferon receptors.	bind
24819	2	6741	5	13	NULL	NULL	NULL	statement 1	Process		phosphorylates					STAT family of transcription factors	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_6_1053_s_188	7586216	16 17 38 39  The fact that the receptor-associated kinases of the JAK family bind to the AT1 receptor and phosphorylate the STAT family of transcription factors 36  suggests that the long-term effects of Ang II on gene expression may resemble those of tyrosine kinase - coupled receptors, such as the PDGF receptor, and classic cytokine receptors, such as the interleukin and interferon receptors.	bind
19350	1	6741	6	NULL	NULL	0	NULL	receptor-associated kinases 	NULL	JAK family	bind	NULL				AT1 receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_77_6_1053_s_188	7586216	16 17 38 39  The fact that the receptor-associated kinases of the JAK family bind to the AT1 receptor and phosphorylate the STAT family of transcription factors 36  suggests that the long-term effects of Ang II on gene expression may resemble those of tyrosine kinase - coupled receptors, such as the PDGF receptor, and classic cytokine receptors, such as the interleukin and interferon receptors.	bind
19351	2	6741	6	10	NULL	0	NULL	statement 1			phosphorylates					STAT family of transcription factors					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_6_1053_s_188	7586216	16 17 38 39  The fact that the receptor-associated kinases of the JAK family bind to the AT1 receptor and phosphorylate the STAT family of transcription factors 36  suggests that the long-term effects of Ang II on gene expression may resemble those of tyrosine kinase - coupled receptors, such as the PDGF receptor, and classic cytokine receptors, such as the interleukin and interferon receptors.	bind
22315	1	6742	5	13	NULL	NULL	NULL	aldosterone	Chemical		bind					MR	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_6_643_s_37	15718497	16 Aldosterone and cortisol bind to human MR with equal affinity.	bind
22323	2	6742	5	13	NULL	NULL	NULL	cortisol	Chemical		bind					MR	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_6_643_s_37	15718497	16 Aldosterone and cortisol bind to human MR with equal affinity.	bind
22325	3	6742	5	13	NULL	NULL	NULL	statement 1	Process		same affinity as					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_6_643_s_37	15718497	16 Aldosterone and cortisol bind to human MR with equal affinity.	bind
19352	1	6742	6	NULL	NULL	0	NULL	aldosterone	NULL		bind	NULL				MR	NULL	human			NULL		0	NULL	NULL	NULL	gw70_circulationres_96_6_643_s_37	15718497	16 Aldosterone and cortisol bind to human MR with equal affinity.	bind
19353	2	6742	6	NULL	NULL	0	NULL	cortisol	NULL		bind	NULL				MR	NULL	human			NULL		0	NULL	NULL	NULL	gw70_circulationres_96_6_643_s_37	15718497	16 Aldosterone and cortisol bind to human MR with equal affinity.	bind
19354	3	6742	6	NULL	NULL	0	NULL	statement 1	NULL		has equal affinity as	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_6_643_s_37	15718497	16 Aldosterone and cortisol bind to human MR with equal affinity.	bind
22324	1	6743	5	13	NULL	NULL	NULL	antibody JTC4	GP		bind					PC	GP		catalytic domain		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_8_865_s_37	12663483	16 Antibody JTC4 binds to the catalytic domain of PC, and its binding to the PC catalytic domain is decreased significantly after reduction.	bind
22328	2	6743	5	13	NULL	NULL	NULL	statement 1	Process		decrease after		significantly			reduction	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_8_865_s_37	12663483	16 Antibody JTC4 binds to the catalytic domain of PC, and its binding to the PC catalytic domain is decreased significantly after reduction.	bind
19355	1	6743	6	NULL	NULL	0	NULL	JTC4 antibody	NULL		bind	NULL				PC	NULL		catalytic domain		NULL		0	NULL	NULL	NULL	gw70_circulationres_92_8_865_s_37	12663483	16 Antibody JTC4 binds to the catalytic domain of PC, and its binding to the PC catalytic domain is decreased significantly after reduction.	bind
56537	2	6743	6	10	NULL	0	NULL	statement 1			decrease after		significantly			reduction					NULL		0	NULL	NULL	NULL	gw70_circulationres_92_8_865_s_37	12663483	16 Antibody JTC4 binds to the catalytic domain of PC, and its binding to the PC catalytic domain is decreased significantly after reduction.	bind
22330	1	6744	5	13	NULL	NULL	NULL	group V sPLA2	GP	human	bind					PC membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_762_s_32	14962950	16 Binding studies using phosphatidylcholine (PC)-coated hydrophobic beads demonstrate that human group V sPLA2 binds PC membranes more than 50-times more tightly than human group IIa sPLA2.	bind
22332	2	6744	5	13	NULL	NULL	NULL	group IIa sPLA2	GP	human	bind					PC membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_762_s_32	14962950	16 Binding studies using phosphatidylcholine (PC)-coated hydrophobic beads demonstrate that human group V sPLA2 binds PC membranes more than 50-times more tightly than human group IIa sPLA2.	bind
22338	3	6744	5	13	NULL	NULL	NULL	statement 1	Process		more tightly than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_762_s_32	14962950	16 Binding studies using phosphatidylcholine (PC)-coated hydrophobic beads demonstrate that human group V sPLA2 binds PC membranes more than 50-times more tightly than human group IIa sPLA2.	bind
19356	1	6744	6	NULL	NULL	0	NULL	group V sPLA2 	NULL	human	bind	NULL				PC membranes	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_762_s_32	14962950	16 Binding studies using phosphatidylcholine (PC)-coated hydrophobic beads demonstrate that human group V sPLA2 binds PC membranes more than 50-times more tightly than human group IIa sPLA2.	bind
19357	2	6744	6	NULL	NULL	0	NULL	group IIa sPLA2	NULL	human	bind	NULL				PC membranes	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_762_s_32	14962950	16 Binding studies using phosphatidylcholine (PC)-coated hydrophobic beads demonstrate that human group V sPLA2 binds PC membranes more than 50-times more tightly than human group IIa sPLA2.	bind
19358	3	6744	6	NULL	NULL	0	NULL	statement 1	NULL		is stronger than	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_762_s_32	14962950	16 Binding studies using phosphatidylcholine (PC)-coated hydrophobic beads demonstrate that human group V sPLA2 binds PC membranes more than 50-times more tightly than human group IIa sPLA2.	bind
22335	1	6745	5	13	NULL	NULL	NULL	Lp-PLA2 plasma isoform	GP		bind					LDL	GP				NULL	in bloodstream	NULL	NULL	NULL	NULL	gw70_circulation_110_14_1903_s_30	15451783	16 In the bloodstream, two thirds of the Lp-PLA2 plasma isoform circulates primarily bound to LDL; the other third is distributed between HDL and VLDL. 17	bind
22336	2	6745	5	13	NULL	NULL	NULL	statement 1	Process		circulates in					blood stream	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_14_1903_s_30	15451783	16 In the bloodstream, two thirds of the Lp-PLA2 plasma isoform circulates primarily bound to LDL; the other third is distributed between HDL and VLDL. 17	bind
19359	1	6745	6	10	NULL	0	NULL	Lp-PLA2 plasma isoform			bind					LDL					NULL	blood stream	NULL	NULL	NULL	NULL	gw70_circulation_110_14_1903_s_30	15451783	16 In the bloodstream, two thirds of the Lp-PLA2 plasma isoform circulates primarily bound to LDL; the other third is distributed between HDL and VLDL. 17	bind
22339	1	6746	5	13	NULL	NULL	NULL	Trx	GP	single mutation at	bind			catalytic site Trx-C32S		ASK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1259_s_257	12089063	16 Our data show that the single mutation of Trx at the catalytic site (Trx-C32S or Trx-C35S) can bind to ASK1, suggesting that the redox activity is not required for the association of Trx with ASK1.	bind
22340	2	6746	5	13	NULL	NULL	NULL	Trx	GP	single mutation at	bind			catalytic site Trx-C35S		ASK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1259_s_257	12089063	16 Our data show that the single mutation of Trx at the catalytic site (Trx-C32S or Trx-C35S) can bind to ASK1, suggesting that the redox activity is not required for the association of Trx with ASK1.	bind
22341	3	6746	5	13	NULL	NULL	NULL	Trx	GP		associates with					ASK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1259_s_257	12089063	16 Our data show that the single mutation of Trx at the catalytic site (Trx-C32S or Trx-C35S) can bind to ASK1, suggesting that the redox activity is not required for the association of Trx with ASK1.	bind
22342	4	6746	5	13	NULL	NULL	NULL	redox activity	Process		is not required for					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1259_s_257	12089063	16 Our data show that the single mutation of Trx at the catalytic site (Trx-C32S or Trx-C35S) can bind to ASK1, suggesting that the redox activity is not required for the association of Trx with ASK1.	bind
56538	5	6746	5	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1259_s_257	12089063	16 Our data show that the single mutation of Trx at the catalytic site (Trx-C32S or Trx-C35S) can bind to ASK1, suggesting that the redox activity is not required for the association of Trx with ASK1.	bind
19360	1	6746	6	10	NULL	0	NULL	Trx		single mutant	bind			catalytic site Trx-C32S		ASK1					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1259_s_257	12089063	16 Our data show that the single mutation of Trx at the catalytic site (Trx-C32S or Trx-C35S) can bind to ASK1, suggesting that the redox activity is not required for the association of Trx with ASK1.	bind
19361	2	6746	6	10	NULL	0	NULL	Trx		single mutant	bind			catalytic site Trx-C35S		ASK1					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1259_s_257	12089063	16 Our data show that the single mutation of Trx at the catalytic site (Trx-C32S or Trx-C35S) can bind to ASK1, suggesting that the redox activity is not required for the association of Trx with ASK1.	bind
19362	3	6746	6	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_12_1259_s_257	12089063	16 Our data show that the single mutation of Trx at the catalytic site (Trx-C32S or Trx-C35S) can bind to ASK1, suggesting that the redox activity is not required for the association of Trx with ASK1.	bind
19363	4	6746	6	NULL	NULL	0	NULL	Trx	NULL	redox activity of	is not required for	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_12_1259_s_257	12089063	16 Our data show that the single mutation of Trx at the catalytic site (Trx-C32S or Trx-C35S) can bind to ASK1, suggesting that the redox activity is not required for the association of Trx with ASK1.	bind
19364	5	6746	6	NULL	NULL	0	NULL	Trx	NULL	redox activity of	is not required for	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_12_1259_s_257	12089063	16 Our data show that the single mutation of Trx at the catalytic site (Trx-C32S or Trx-C35S) can bind to ASK1, suggesting that the redox activity is not required for the association of Trx with ASK1.	bind
22343	1	6747	5	13	NULL	NULL	NULL	APOA5	GP		is					apolipoprotein A-V	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_9_1985_s_38	15976322	16 Recently USF1 was also shown to stimulate apolipoprotein A-V ( APOA5) promoter activity in an insulin-dependent manner, demonstrated by the reduced binding of USF1 to the  APOA5 promoter in the presence of insulin.	bind
22344	2	6747	5	13	NULL	NULL	NULL	USF1	GP		bind					APOA5	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_9_1985_s_38	15976322	16 Recently USF1 was also shown to stimulate apolipoprotein A-V ( APOA5) promoter activity in an insulin-dependent manner, demonstrated by the reduced binding of USF1 to the  APOA5 promoter in the presence of insulin.	bind
22345	3	6747	5	13	NULL	NULL	NULL	insulin	GP		reduces					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_9_1985_s_38	15976322	16 Recently USF1 was also shown to stimulate apolipoprotein A-V ( APOA5) promoter activity in an insulin-dependent manner, demonstrated by the reduced binding of USF1 to the  APOA5 promoter in the presence of insulin.	bind
22346	4	6747	5	13	NULL	NULL	NULL	USF1	GP		stimulates					APOA5	GP	activity of		promoter	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_9_1985_s_38	15976322	16 Recently USF1 was also shown to stimulate apolipoprotein A-V ( APOA5) promoter activity in an insulin-dependent manner, demonstrated by the reduced binding of USF1 to the  APOA5 promoter in the presence of insulin.	bind
22347	5	6747	5	13	NULL	NULL	NULL	statement 4	Process		is dependent on					insulin	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_9_1985_s_38	15976322	16 Recently USF1 was also shown to stimulate apolipoprotein A-V ( APOA5) promoter activity in an insulin-dependent manner, demonstrated by the reduced binding of USF1 to the  APOA5 promoter in the presence of insulin.	bind
19365	1	6747	6	NULL	NULL	0	NULL	USF1	NULL		bind	NULL				APOA5	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_9_1985_s_38	15976322	16 Recently USF1 was also shown to stimulate apolipoprotein A-V ( APOA5) promoter activity in an insulin-dependent manner, demonstrated by the reduced binding of USF1 to the  APOA5 promoter in the presence of insulin.	bind
19366	2	6747	6	NULL	NULL	0	NULL	APOA5	NULL		is	NULL				apolipoprotein A-V	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_9_1985_s_38	15976322	16 Recently USF1 was also shown to stimulate apolipoprotein A-V ( APOA5) promoter activity in an insulin-dependent manner, demonstrated by the reduced binding of USF1 to the  APOA5 promoter in the presence of insulin.	bind
19367	3	6747	6	10	NULL	0	NULL	insulin			reduces					statement 1					NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_9_1985_s_38	15976322	16 Recently USF1 was also shown to stimulate apolipoprotein A-V ( APOA5) promoter activity in an insulin-dependent manner, demonstrated by the reduced binding of USF1 to the  APOA5 promoter in the presence of insulin.	bind
56539	4	6747	6	10	NULL	0	NULL	USF1			stimulate					APOA5		activity of		promoter	NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_9_1985_s_38	15976322	16 Recently USF1 was also shown to stimulate apolipoprotein A-V ( APOA5) promoter activity in an insulin-dependent manner, demonstrated by the reduced binding of USF1 to the  APOA5 promoter in the presence of insulin.	bind
56540	5	6747	6	10	NULL	0	NULL	statement 4			depends on					insulin					NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_9_1985_s_38	15976322	16 Recently USF1 was also shown to stimulate apolipoprotein A-V ( APOA5) promoter activity in an insulin-dependent manner, demonstrated by the reduced binding of USF1 to the  APOA5 promoter in the presence of insulin.	bind
22348	1	6748	5	13	NULL	NULL	NULL	L22 protein	GP		bind		primarily			23S rRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jantimicrobchemoth_52_3_345_s_303	12917252	16 The L22 protein binds primarily to the 23S rRNA.	bind
19368	1	6748	6	NULL	NULL	0	NULL	L22 protein	NULL		bind	NULL	primarily			23S rRNA	NULL				NULL		0	NULL	NULL	NULL	gw70_jantimicrobchemoth_52_3_345_s_303	12917252	16 The L22 protein binds primarily to the 23S rRNA.	bind
22350	1	6749	5	13	NULL	NULL	NULL	PDGF-BB	GP		bind					R-1 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_15_1830_s_92	11956127	16 There were no differences in PDGF-BB binding to R-1, R-2, and C-1 cells or the levels of immunoreactive PDGF-beta receptor among these cells ( Figure 3A).	bind
22351	2	6749	5	13	NULL	NULL	NULL	PDGF-BB	GP		bind					R-2 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_15_1830_s_92	11956127	16 There were no differences in PDGF-BB binding to R-1, R-2, and C-1 cells or the levels of immunoreactive PDGF-beta receptor among these cells ( Figure 3A).	bind
22352	3	6749	5	13	NULL	NULL	NULL	PDGF-BB	GP		bind					C-1 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_15_1830_s_92	11956127	16 There were no differences in PDGF-BB binding to R-1, R-2, and C-1 cells or the levels of immunoreactive PDGF-beta receptor among these cells ( Figure 3A).	bind
19369	1	6749	6	NULL	NULL	0	NULL	PDGF-BB	NULL		bind	NULL				R-1 cells	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_15_1830_s_92	11956127	16 There were no differences in PDGF-BB binding to R-1, R-2, and C-1 cells or the levels of immunoreactive PDGF-beta receptor among these cells ( Figure 3A).	bind
19370	2	6749	6	NULL	NULL	0	NULL	PDGF-BB	NULL		bind	NULL				R-2 cells	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_15_1830_s_92	11956127	16 There were no differences in PDGF-BB binding to R-1, R-2, and C-1 cells or the levels of immunoreactive PDGF-beta receptor among these cells ( Figure 3A).	bind
19371	3	6749	6	NULL	NULL	0	NULL	PDGF-BB	NULL		bind	NULL				C-1 cells	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_15_1830_s_92	11956127	16 There were no differences in PDGF-BB binding to R-1, R-2, and C-1 cells or the levels of immunoreactive PDGF-beta receptor among these cells ( Figure 3A).	bind
22353	1	6750	5	13	NULL	NULL	NULL	TIMPs	GP		bind					MMPs	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_9_1166_s_31	15723986	16 TIMPs bind to MMPs in a 1:1 ratio, thereby preventing continued proteolytic activity.	bind
22354	2	6750	5	13	NULL	NULL	NULL	statement 1	Process		prevents					proteolytic activity	Process	continued			NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_9_1166_s_31	15723986	16 TIMPs bind to MMPs in a 1:1 ratio, thereby preventing continued proteolytic activity.	bind
19372	1	6750	6	NULL	NULL	0	NULL	TIMP	NULL		bind	NULL				MMP	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_111_9_1166_s_31	15723986	16 TIMPs bind to MMPs in a 1:1 ratio, thereby preventing continued proteolytic activity.	bind
56541	2	6750	6	10	NULL	0	NULL	statement 1			prevents					proteolytic activity		continued			NULL		0	NULL	NULL	NULL	gw70_circulation_111_9_1166_s_31	15723986	16 TIMPs bind to MMPs in a 1:1 ratio, thereby preventing continued proteolytic activity.	bind
22355	1	6751	5	13	NULL	NULL	NULL	fibrinogen	GP		bind					GP IIb/IIa receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1720_s_30	15242858	16 VASP phosphorylation correlates closely with inhibition of fibrinogen binding to the GP IIb/IIa receptor.	bind
22356	2	6751	5	13	NULL	NULL	NULL	VASP	GP	phosphorylation	correlates with		closely			statement 1	Process	inhibition of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1720_s_30	15242858	16 VASP phosphorylation correlates closely with inhibition of fibrinogen binding to the GP IIb/IIa receptor.	bind
19373	1	6751	6	NULL	NULL	0	NULL	fibrinogen	NULL		bind	NULL				GP IIb/IIa receptor	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1720_s_30	15242858	16 VASP phosphorylation correlates closely with inhibition of fibrinogen binding to the GP IIb/IIa receptor.	bind
19374	2	6751	6	NULL	NULL	0	NULL	VASP	NULL	phosphorylation of	correlates with	NULL				statement 1	NULL	inhibition of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1720_s_30	15242858	16 VASP phosphorylation correlates closely with inhibition of fibrinogen binding to the GP IIb/IIa receptor.	bind
22357	1	6753	5	13	NULL	NULL	NULL	growth factor	GP		bind					receptor tyrosine kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_3_899_s_15	10079268	16, 17  It is believed that the initial events involve binding of growth factor to a receptor tyrosine kinase and receptor oligomerization.	bind
22358	2	6753	5	13	NULL	NULL	NULL	statement 1	Process		leads to					receptor 	GP	oligomerization of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_3_899_s_15	10079268	16, 17  It is believed that the initial events involve binding of growth factor to a receptor tyrosine kinase and receptor oligomerization.	bind
19375	1	6753	6	NULL	NULL	0	NULL	growth factor	NULL		bind	NULL				receptor tyrosine kinase	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_3_899_s_15	10079268	16, 17  It is believed that the initial events involve binding of growth factor to a receptor tyrosine kinase and receptor oligomerization.	bind
56542	2	6753	6	10	NULL	0	NULL	statement 1			leads to					receptor		oligomerization of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_3_899_s_15	10079268	16, 17  It is believed that the initial events involve binding of growth factor to a receptor tyrosine kinase and receptor oligomerization.	bind
22359	1	6754	5	13	NULL	NULL	NULL	IL-6	GP	murine	does not bind					IL-6R	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_2_639_s_20	9708822	16, 17  Transgenic mice expressing the human sIL-6R do not develop any specific morphological changes, because murine IL-6 does not bind to the human IL-6R.	bind
19376	1	6754	6	NULL	NULL	0	NULL	IL-6	NULL	murine	does not bind	NULL				IL-6R	NULL	human			NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_2_639_s_20	9708822	16, 17  Transgenic mice expressing the human sIL-6R do not develop any specific morphological changes, because murine IL-6 does not bind to the human IL-6R.	bind
22360	1	6755	5	13	NULL	NULL	NULL	alpha1	GP		bind			I domain		type II collagen	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1779_s_20	12000729	16, 17 Thus, although alpha1 I domain can bind type II collagen and the alpha1 integrin can probably transduce signals from type II collagen, it is likely that adhesion to type II collagen of structural importance is mediated by alpha2beta1.	bind
22361	2	6755	5	13	NULL	NULL	NULL	alpha1 integrin	GP		transduce		probably			type II collagen	GP	signals from			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1779_s_20	12000729	16, 17 Thus, although alpha1 I domain can bind type II collagen and the alpha1 integrin can probably transduce signals from type II collagen, it is likely that adhesion to type II collagen of structural importance is mediated by alpha2beta1.	bind
22362	3	6755	5	13	NULL	NULL	NULL	type II collagen	GP	adhesion to	is mediated by					alpha2beta1	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1779_s_20	12000729	16, 17 Thus, although alpha1 I domain can bind type II collagen and the alpha1 integrin can probably transduce signals from type II collagen, it is likely that adhesion to type II collagen of structural importance is mediated by alpha2beta1.	bind
19528	1	6755	6	10	NULL	0	NULL	alpha1			bind			 I domain		type II collagen					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1779_s_20	12000729	16, 17 Thus, although alpha1 I domain can bind type II collagen and the alpha1 integrin can probably transduce signals from type II collagen, it is likely that adhesion to type II collagen of structural importance is mediated by alpha2beta1.	bind
19529	2	6755	6	NULL	NULL	0	NULL	alpha2beta1	NULL		mediates	NULL				type II collagen	NULL	adhesion to			NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_5_1779_s_20	12000729	16, 17 Thus, although alpha1 I domain can bind type II collagen and the alpha1 integrin can probably transduce signals from type II collagen, it is likely that adhesion to type II collagen of structural importance is mediated by alpha2beta1.	bind
19530	3	6755	6	NULL	NULL	0	NULL	alpha1 integrin	NULL		transduce	NULL	probably			type II collagen	NULL	signals from			NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_5_1779_s_20	12000729	16, 17 Thus, although alpha1 I domain can bind type II collagen and the alpha1 integrin can probably transduce signals from type II collagen, it is likely that adhesion to type II collagen of structural importance is mediated by alpha2beta1.	bind
22363	1	6756	5	13	NULL	NULL	NULL	ALK	GP		interacts with					PLC-gamma	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_3_875_s_187	12213716	16, 19, 20  Further, the interaction between ALK and PLC-gamma has been shown to be essential because mutation of the ALK residue responsible for PLC-gamma binding eliminates the transforming potential of NPM-ALK.	bind
22364	3	6756	5	13	NULL	NULL	NULL	statement 2	Process		eliminates					NPM-ALK	GP	transforming potential of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_3_875_s_187	12213716	16, 19, 20  Further, the interaction between ALK and PLC-gamma has been shown to be essential because mutation of the ALK residue responsible for PLC-gamma binding eliminates the transforming potential of NPM-ALK.	bind
44688	2	6756	5	13	NULL	NULL	NULL			mutation of	responsible for			ALK residue		PLC-gamma	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_3_875_s_187	12213716	16, 19, 20  Further, the interaction between ALK and PLC-gamma has been shown to be essential because mutation of the ALK residue responsible for PLC-gamma binding eliminates the transforming potential of NPM-ALK.	bind
19531	1	6756	6	NULL	NULL	0	NULL	ALK	NULL		interacts with	NULL				PLC-gamma	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_3_875_s_187	12213716	16, 19, 20  Further, the interaction between ALK and PLC-gamma has been shown to be essential because mutation of the ALK residue responsible for PLC-gamma binding eliminates the transforming potential of NPM-ALK.	bind
19532	2	6756	6	10	NULL	0	NULL	ALK		mutant	responsible for					PLC-gamma		binding of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_3_875_s_187	12213716	16, 19, 20  Further, the interaction between ALK and PLC-gamma has been shown to be essential because mutation of the ALK residue responsible for PLC-gamma binding eliminates the transforming potential of NPM-ALK.	bind
56543	3	6756	6	10	NULL	0	NULL	statement 2			eliminates					NPM-ALK		transforming potential of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_3_875_s_187	12213716	16, 19, 20  Further, the interaction between ALK and PLC-gamma has been shown to be essential because mutation of the ALK residue responsible for PLC-gamma binding eliminates the transforming potential of NPM-ALK.	bind
22365	1	6757	5	13	NULL	NULL	NULL	P300	GP		bind					transactivator-DNA complex	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_23_2760_s_160	12057991	16, 25 In this study, we provide direct evidence for P300 binding to transactivator-DNA complex.	bind
19533	1	6757	6	NULL	NULL	0	NULL	p300	NULL		bind	NULL	directly			transactivator-DNA complex	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_23_2760_s_160	12057991	16, 25 In this study, we provide direct evidence for P300 binding to transactivator-DNA complex.	bind
22366	1	6758	5	13	NULL	NULL	NULL	apoptotic protease-activating factor 1	GP		bind					ADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_nature_442_7098_39_s_228	16823444	16, 48-62 (2004) |  Article |  PubMed |  ISI |  ChemPort |    iedl, S. J. ,  Li, W. ,  Chao, Y. ,  Schwarzenbacher, [[ R.  &  Shi ]], Y.  Structure  of the apoptotic protease-activating factor 1 bound to ADP.	bind
19534	1	6758	6	10	NULL	0	NULL	apoptotic protease-activating factor 1	NULL		bind	NULL				ADP	NULL				NULL		NULL	NULL	NULL	NULL	gw70_nature_442_7098_39_s_228	16823444	16, 48-62 (2004) |  Article |  PubMed |  ISI |  ChemPort |    iedl, S. J. ,  Li, W. ,  Chao, Y. ,  Schwarzenbacher, [[ R.  &  Shi ]], Y.  Structure  of the apoptotic protease-activating factor 1 bound to ADP.	bind
22367	1	6760	5	13	NULL	NULL	NULL	Hip	GP		bind					Hsc70	GP		ATPase domain		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_100	9686751	166 247 248  After Hsp40 is released, Hip binds to the ATPase domain of Hsc70 (E), stimulates its activity, and then remains bound to stabilize the ADP-Hsc70-substrate complex, suggesting that it may play a role in the transport of substrates within cells (F).	bind
22368	2	6760	5	13	NULL	NULL	NULL	statement 1	Process		occurs after					Hsp40	GP	release of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_100	9686751	166 247 248  After Hsp40 is released, Hip binds to the ATPase domain of Hsc70 (E), stimulates its activity, and then remains bound to stabilize the ADP-Hsc70-substrate complex, suggesting that it may play a role in the transport of substrates within cells (F).	bind
22369	3	6760	5	13	NULL	NULL	NULL	statement 1	Process		stimulates					Hsc70	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_100	9686751	166 247 248  After Hsp40 is released, Hip binds to the ATPase domain of Hsc70 (E), stimulates its activity, and then remains bound to stabilize the ADP-Hsc70-substrate complex, suggesting that it may play a role in the transport of substrates within cells (F).	bind
22370	4	6760	5	13	NULL	NULL	NULL	Hip	GP		remains					Hsc70	GP	bound to			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_100	9686751	166 247 248  After Hsp40 is released, Hip binds to the ATPase domain of Hsc70 (E), stimulates its activity, and then remains bound to stabilize the ADP-Hsc70-substrate complex, suggesting that it may play a role in the transport of substrates within cells (F).	bind
22371	5	6760	5	13	NULL	NULL	NULL	statement 4	Process		stabilizes					ADP-Hsc70-substrate complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_100	9686751	166 247 248  After Hsp40 is released, Hip binds to the ATPase domain of Hsc70 (E), stimulates its activity, and then remains bound to stabilize the ADP-Hsc70-substrate complex, suggesting that it may play a role in the transport of substrates within cells (F).	bind
22372	6	6760	5	13	NULL	NULL	NULL	statement 5	Process		plays a role in		may			substrates	GP	transport of			NULL	within cells	NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_100	9686751	166 247 248  After Hsp40 is released, Hip binds to the ATPase domain of Hsc70 (E), stimulates its activity, and then remains bound to stabilize the ADP-Hsc70-substrate complex, suggesting that it may play a role in the transport of substrates within cells (F).	bind
19535	1	6760	6	NULL	NULL	0	NULL	Hip	NULL		bind	NULL				Hsc70	NULL		ATPase domain		NULL		0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_100	9686751	166 247 248  After Hsp40 is released, Hip binds to the ATPase domain of Hsc70 (E), stimulates its activity, and then remains bound to stabilize the ADP-Hsc70-substrate complex, suggesting that it may play a role in the transport of substrates within cells (F).	bind
19536	2	6760	6	10	NULL	0	NULL	statement 1			occurs after 		release of			Hsp40					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_100	9686751	166 247 248  After Hsp40 is released, Hip binds to the ATPase domain of Hsc70 (E), stimulates its activity, and then remains bound to stabilize the ADP-Hsc70-substrate complex, suggesting that it may play a role in the transport of substrates within cells (F).	bind
19537	3	6760	6	NULL	NULL	0	NULL	Hip	NULL		stimulates 	NULL				Hsc70	NULL	activity of 			NULL		0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_100	9686751	166 247 248  After Hsp40 is released, Hip binds to the ATPase domain of Hsc70 (E), stimulates its activity, and then remains bound to stabilize the ADP-Hsc70-substrate complex, suggesting that it may play a role in the transport of substrates within cells (F).	bind
19538	4	6760	6	NULL	NULL	0	NULL	ADP	NULL		forms a complex with	NULL				Hsc70	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_100	9686751	166 247 248  After Hsp40 is released, Hip binds to the ATPase domain of Hsc70 (E), stimulates its activity, and then remains bound to stabilize the ADP-Hsc70-substrate complex, suggesting that it may play a role in the transport of substrates within cells (F).	bind
19539	5	6760	6	NULL	NULL	0	NULL	Hip	NULL		stabilizes	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_100	9686751	166 247 248  After Hsp40 is released, Hip binds to the ATPase domain of Hsc70 (E), stimulates its activity, and then remains bound to stabilize the ADP-Hsc70-substrate complex, suggesting that it may play a role in the transport of substrates within cells (F).	bind
19540	6	6760	6	NULL	NULL	0	NULL	Hip	NULL		plays a role in	NULL	may			substrates	NULL	transport of 			NULL	cells	0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_100	9686751	166 247 248  After Hsp40 is released, Hip binds to the ATPase domain of Hsc70 (E), stimulates its activity, and then remains bound to stabilize the ADP-Hsc70-substrate complex, suggesting that it may play a role in the transport of substrates within cells (F).	bind
23224	1	6761	5	13	NULL	NULL	NULL	XPG	GP		bind					PCNA	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_6_1341_s_359	11239001	17       Gary,R., Ludwig,D.L., Cornelius,H.L., MacInnes,M.A. and Park,M.S. (1997) The DNA repair endonuclease XPG binds to proliferating cell nuclear antigen (PCNA) and shares sequence elements with the PCNA-binding regions of FEN-1 and cyclin-dependent kinase inhibitor p21.	bind
23225	2	6761	5	13	NULL	NULL	NULL	XPG	GP		is a type of					DNA repair endonuclease	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_6_1341_s_359	11239001	17       Gary,R., Ludwig,D.L., Cornelius,H.L., MacInnes,M.A. and Park,M.S. (1997) The DNA repair endonuclease XPG binds to proliferating cell nuclear antigen (PCNA) and shares sequence elements with the PCNA-binding regions of FEN-1 and cyclin-dependent kinase inhibitor p21.	bind
23226	3	6761	5	13	NULL	NULL	NULL	PCNA	GP		is					proliferating cell nuclear antigen	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_6_1341_s_359	11239001	17       Gary,R., Ludwig,D.L., Cornelius,H.L., MacInnes,M.A. and Park,M.S. (1997) The DNA repair endonuclease XPG binds to proliferating cell nuclear antigen (PCNA) and shares sequence elements with the PCNA-binding regions of FEN-1 and cyclin-dependent kinase inhibitor p21.	bind
23227	4	6761	5	13	NULL	NULL	NULL	XPG	GP		share					FEN-1	GP	sequence elements with	PCNA-binding regions		NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_6_1341_s_359	11239001	17       Gary,R., Ludwig,D.L., Cornelius,H.L., MacInnes,M.A. and Park,M.S. (1997) The DNA repair endonuclease XPG binds to proliferating cell nuclear antigen (PCNA) and shares sequence elements with the PCNA-binding regions of FEN-1 and cyclin-dependent kinase inhibitor p21.	bind
23228	5	6761	5	13	NULL	NULL	NULL	XPG	GP		share					p21	GP	sequence elements with			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_6_1341_s_359	11239001	17       Gary,R., Ludwig,D.L., Cornelius,H.L., MacInnes,M.A. and Park,M.S. (1997) The DNA repair endonuclease XPG binds to proliferating cell nuclear antigen (PCNA) and shares sequence elements with the PCNA-binding regions of FEN-1 and cyclin-dependent kinase inhibitor p21.	bind
23230	6	6761	5	13	NULL	NULL	NULL	p21	GP		is a type of					cyclin-dependent kinase inhibitor	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_6_1341_s_359	11239001	17       Gary,R., Ludwig,D.L., Cornelius,H.L., MacInnes,M.A. and Park,M.S. (1997) The DNA repair endonuclease XPG binds to proliferating cell nuclear antigen (PCNA) and shares sequence elements with the PCNA-binding regions of FEN-1 and cyclin-dependent kinase inhibitor p21.	bind
19541	1	6761	6	10	NULL	0	NULL	XPG	NULL		is a type of	NULL				DNA repair endonuclease	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_6_1341_s_359	11239001	17       Gary,R., Ludwig,D.L., Cornelius,H.L., MacInnes,M.A. and Park,M.S. (1997) The DNA repair endonuclease XPG binds to proliferating cell nuclear antigen (PCNA) and shares sequence elements with the PCNA-binding regions of FEN-1 and cyclin-dependent kinase inhibitor p21.	bind
19542	2	6761	6	NULL	NULL	0	NULL	XPG	NULL		bind	NULL				PCNA	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_6_1341_s_359	11239001	17       Gary,R., Ludwig,D.L., Cornelius,H.L., MacInnes,M.A. and Park,M.S. (1997) The DNA repair endonuclease XPG binds to proliferating cell nuclear antigen (PCNA) and shares sequence elements with the PCNA-binding regions of FEN-1 and cyclin-dependent kinase inhibitor p21.	bind
19543	3	6761	6	NULL	NULL	0	NULL	PCNA	NULL		is	NULL				proliferating cell nuclear antigen	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_6_1341_s_359	11239001	17       Gary,R., Ludwig,D.L., Cornelius,H.L., MacInnes,M.A. and Park,M.S. (1997) The DNA repair endonuclease XPG binds to proliferating cell nuclear antigen (PCNA) and shares sequence elements with the PCNA-binding regions of FEN-1 and cyclin-dependent kinase inhibitor p21.	bind
56544	4	6761	6	10	NULL	0	NULL	XPG			shares					FEN-1		sequence elements with	PCNA-binding region		NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_6_1341_s_359	11239001	17       Gary,R., Ludwig,D.L., Cornelius,H.L., MacInnes,M.A. and Park,M.S. (1997) The DNA repair endonuclease XPG binds to proliferating cell nuclear antigen (PCNA) and shares sequence elements with the PCNA-binding regions of FEN-1 and cyclin-dependent kinase inhibitor p21.	bind
56545	5	6761	6	10	NULL	0	NULL	XPG			shares					p21		sequence elements with			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_6_1341_s_359	11239001	17       Gary,R., Ludwig,D.L., Cornelius,H.L., MacInnes,M.A. and Park,M.S. (1997) The DNA repair endonuclease XPG binds to proliferating cell nuclear antigen (PCNA) and shares sequence elements with the PCNA-binding regions of FEN-1 and cyclin-dependent kinase inhibitor p21.	bind
56546	6	6761	6	10	NULL	0	NULL	p21			is a type of					cyclin-dependent kinase inhibitor					NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_6_1341_s_359	11239001	17       Gary,R., Ludwig,D.L., Cornelius,H.L., MacInnes,M.A. and Park,M.S. (1997) The DNA repair endonuclease XPG binds to proliferating cell nuclear antigen (PCNA) and shares sequence elements with the PCNA-binding regions of FEN-1 and cyclin-dependent kinase inhibitor p21.	bind
23231	1	6763	5	13	NULL	NULL	NULL	Cu2+	Chemical		bind					LDL	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3338_s_35	9409331	17  19  Subsequent studies have shown that Cu2+ binds to LDL 20 21  22  and that LDL can reduce Cu2+ to Cu1+.	bind
23232	2	6763	5	13	NULL	NULL	NULL	Cu2+	Chemical		is reduced to					Cu1+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3338_s_35	9409331	17  19  Subsequent studies have shown that Cu2+ binds to LDL 20 21  22  and that LDL can reduce Cu2+ to Cu1+.	bind
23233	3	6763	5	13	NULL	NULL	NULL	LDL	GP		is required for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3338_s_35	9409331	17  19  Subsequent studies have shown that Cu2+ binds to LDL 20 21  22  and that LDL can reduce Cu2+ to Cu1+.	bind
19546	1	6763	6	NULL	NULL	0	NULL	Cu2+	NULL		bind	NULL				LDL	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3338_s_35	9409331	17  19  Subsequent studies have shown that Cu2+ binds to LDL 20 21  22  and that LDL can reduce Cu2+ to Cu1+.	bind
19547	2	6763	6	NULL	NULL	0	NULL	Cu2+	NULL		reduced to	NULL				Cu1+	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3338_s_35	9409331	17  19  Subsequent studies have shown that Cu2+ binds to LDL 20 21  22  and that LDL can reduce Cu2+ to Cu1+.	bind
19548	3	6763	6	NULL	NULL	0	NULL	statement 2	NULL		occurs by	NULL				LDL	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3338_s_35	9409331	17  19  Subsequent studies have shown that Cu2+ binds to LDL 20 21  22  and that LDL can reduce Cu2+ to Cu1+.	bind
23234	1	6764	5	13	NULL	NULL	NULL	vWF	GP		is changed to			RDDS		vWF	GP		RGGS		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_6_1661_s_43	10845886	17  Arg-Gly-Gly-Ser (RGGS)-vWF, in which Asp (D)-1746 has been changed to Gly (G), has virtually no binding to thrombin-stimulated platelets, indicating that the interaction of this vWF with alphaIIb-beta3 is defective.	bind
23235	2	6764	5	13	NULL	NULL	NULL	statement 1	GP		does not bind					platelets	Cell	thrombin-stimulated			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_6_1661_s_43	10845886	17  Arg-Gly-Gly-Ser (RGGS)-vWF, in which Asp (D)-1746 has been changed to Gly (G), has virtually no binding to thrombin-stimulated platelets, indicating that the interaction of this vWF with alphaIIb-beta3 is defective.	bind
23236	3	6764	5	13	NULL	NULL	NULL	vWF	GP		interacts with					alphaIIb-beta3	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_6_1661_s_43	10845886	17  Arg-Gly-Gly-Ser (RGGS)-vWF, in which Asp (D)-1746 has been changed to Gly (G), has virtually no binding to thrombin-stimulated platelets, indicating that the interaction of this vWF with alphaIIb-beta3 is defective.	bind
23237	4	6764	5	13	NULL	NULL	NULL	statement 2	Process		indicates					statement 3	Process	defective			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_6_1661_s_43	10845886	17  Arg-Gly-Gly-Ser (RGGS)-vWF, in which Asp (D)-1746 has been changed to Gly (G), has virtually no binding to thrombin-stimulated platelets, indicating that the interaction of this vWF with alphaIIb-beta3 is defective.	bind
19818	2	6764	6	10	NULL	0	NULL	statement 1			does not bind					platelets		thrombin-stimulated			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_6_1661_s_43	10845886	17  Arg-Gly-Gly-Ser (RGGS)-vWF, in which Asp (D)-1746 has been changed to Gly (G), has virtually no binding to thrombin-stimulated platelets, indicating that the interaction of this vWF with alphaIIb-beta3 is defective.	bind
19819	3	6764	6	10	NULL	0	NULL	vWF 			 interact with					alphaIIb-beta3					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_6_1661_s_43	10845886	17  Arg-Gly-Gly-Ser (RGGS)-vWF, in which Asp (D)-1746 has been changed to Gly (G), has virtually no binding to thrombin-stimulated platelets, indicating that the interaction of this vWF with alphaIIb-beta3 is defective.	bind
19820	4	6764	6	10	NULL	0	NULL	statement 2			indicates					statement 3		defective			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_6_1661_s_43	10845886	17  Arg-Gly-Gly-Ser (RGGS)-vWF, in which Asp (D)-1746 has been changed to Gly (G), has virtually no binding to thrombin-stimulated platelets, indicating that the interaction of this vWF with alphaIIb-beta3 is defective.	bind
56547	1	6764	6	10	NULL	0	NULL	vWF			is changed to			RDDS		vWF			RGGS		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_6_1661_s_43	10845886	17  Arg-Gly-Gly-Ser (RGGS)-vWF, in which Asp (D)-1746 has been changed to Gly (G), has virtually no binding to thrombin-stimulated platelets, indicating that the interaction of this vWF with alphaIIb-beta3 is defective.	bind
23238	1	6765	5	13	NULL	NULL	NULL	anti-hsp65/60 Abs	GP	serum	bind		high affinity			GroEL	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_3_536_s_151	9102173	17  As a consequence of this and because serum anti-hsp65/60 Abs also exhibit a high binding capacity to GroEL, the corresponding areas of Ab binding on the three-dimensional GroEL structure may be of interest.	bind
19549	1	6765	6	NULL	NULL	0	NULL	anti-hsp65/60 Abs	NULL	serum	bind	NULL	high affinity			GroEL	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_3_536_s_151	9102173	17  As a consequence of this and because serum anti-hsp65/60 Abs also exhibit a high binding capacity to GroEL, the corresponding areas of Ab binding on the three-dimensional GroEL structure may be of interest.	bind
23239	1	6766	5	13	NULL	NULL	NULL	perlecan	GP		bind			core protein		Abeta 	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2115_s_21	10595940	17  Because perlecan can bind to both Abeta and the amyloid precursor protein (betaPP) through its core protein or GAG moieties, 18- 21  this molecule may play a significant role in amyloid formation in Alzheimer s disease, eg, by affecting the processing of betaPP or by determining the localization of Abeta deposition at sites where perlecan is produced.	bind
23244	2	6766	5	13	NULL	NULL	NULL	perlecan	GP		bind			GAG moieties		Abeta	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2115_s_21	10595940	17  Because perlecan can bind to both Abeta and the amyloid precursor protein (betaPP) through its core protein or GAG moieties, 18- 21  this molecule may play a significant role in amyloid formation in Alzheimer s disease, eg, by affecting the processing of betaPP or by determining the localization of Abeta deposition at sites where perlecan is produced.	bind
23245	3	6766	5	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2115_s_21	10595940	17  Because perlecan can bind to both Abeta and the amyloid precursor protein (betaPP) through its core protein or GAG moieties, 18- 21  this molecule may play a significant role in amyloid formation in Alzheimer s disease, eg, by affecting the processing of betaPP or by determining the localization of Abeta deposition at sites where perlecan is produced.	bind
23246	4	6766	5	13	NULL	NULL	NULL	betaPP	GP		is a type of					amyloid precursor protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2115_s_21	10595940	17  Because perlecan can bind to both Abeta and the amyloid precursor protein (betaPP) through its core protein or GAG moieties, 18- 21  this molecule may play a significant role in amyloid formation in Alzheimer s disease, eg, by affecting the processing of betaPP or by determining the localization of Abeta deposition at sites where perlecan is produced.	bind
23247	5	6766	5	13	NULL	NULL	NULL	perlecan	GP		bind			core protein		betaPP	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2115_s_21	10595940	17  Because perlecan can bind to both Abeta and the amyloid precursor protein (betaPP) through its core protein or GAG moieties, 18- 21  this molecule may play a significant role in amyloid formation in Alzheimer s disease, eg, by affecting the processing of betaPP or by determining the localization of Abeta deposition at sites where perlecan is produced.	bind
23248	6	6766	5	13	NULL	NULL	NULL	perlecan	GP		bind			GAG moieties		betaPP	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2115_s_21	10595940	17  Because perlecan can bind to both Abeta and the amyloid precursor protein (betaPP) through its core protein or GAG moieties, 18- 21  this molecule may play a significant role in amyloid formation in Alzheimer s disease, eg, by affecting the processing of betaPP or by determining the localization of Abeta deposition at sites where perlecan is produced.	bind
23249	7	6766	5	13	NULL	NULL	NULL	statement 5	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2115_s_21	10595940	17  Because perlecan can bind to both Abeta and the amyloid precursor protein (betaPP) through its core protein or GAG moieties, 18- 21  this molecule may play a significant role in amyloid formation in Alzheimer s disease, eg, by affecting the processing of betaPP or by determining the localization of Abeta deposition at sites where perlecan is produced.	bind
23250	8	6766	5	13	NULL	NULL	NULL	perlecan	GP		plays a role in		may;;significant			amyloid	GP	formation of			NULL	in Alzheimer s disease	NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2115_s_21	10595940	17  Because perlecan can bind to both Abeta and the amyloid precursor protein (betaPP) through its core protein or GAG moieties, 18- 21  this molecule may play a significant role in amyloid formation in Alzheimer s disease, eg, by affecting the processing of betaPP or by determining the localization of Abeta deposition at sites where perlecan is produced.	bind
23251	9	6766	5	13	NULL	NULL	NULL	perlecan	GP		affect					betaPP	GP	processing of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2115_s_21	10595940	17  Because perlecan can bind to both Abeta and the amyloid precursor protein (betaPP) through its core protein or GAG moieties, 18- 21  this molecule may play a significant role in amyloid formation in Alzheimer s disease, eg, by affecting the processing of betaPP or by determining the localization of Abeta deposition at sites where perlecan is produced.	bind
19550	1	6766	6	NULL	NULL	0	NULL	perlecan	NULL		bind	NULL		GAG moeity		Abeta	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2115_s_21	10595940	17  Because perlecan can bind to both Abeta and the amyloid precursor protein (betaPP) through its core protein or GAG moieties, 18- 21  this molecule may play a significant role in amyloid formation in Alzheimer s disease, eg, by affecting the processing of betaPP or by determining the localization of Abeta deposition at sites where perlecan is produced.	bind
19551	2	6766	6	NULL	NULL	0	NULL	perlecan	NULL		bind	NULL		GAG moeity		betaPP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2115_s_21	10595940	17  Because perlecan can bind to both Abeta and the amyloid precursor protein (betaPP) through its core protein or GAG moieties, 18- 21  this molecule may play a significant role in amyloid formation in Alzheimer s disease, eg, by affecting the processing of betaPP or by determining the localization of Abeta deposition at sites where perlecan is produced.	bind
19552	3	6766	6	10	NULL	0	NULL	betaPP			is a type of					amyloid precursor protein					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2115_s_21	10595940	17  Because perlecan can bind to both Abeta and the amyloid precursor protein (betaPP) through its core protein or GAG moieties, 18- 21  this molecule may play a significant role in amyloid formation in Alzheimer s disease, eg, by affecting the processing of betaPP or by determining the localization of Abeta deposition at sites where perlecan is produced.	bind
19553	4	6766	6	10	NULL	0	NULL	perlecan			play a role in		may			amyloid 		formation of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2115_s_21	10595940	17  Because perlecan can bind to both Abeta and the amyloid precursor protein (betaPP) through its core protein or GAG moieties, 18- 21  this molecule may play a significant role in amyloid formation in Alzheimer s disease, eg, by affecting the processing of betaPP or by determining the localization of Abeta deposition at sites where perlecan is produced.	bind
19554	5	6766	6	NULL	NULL	0	NULL	statement 4	NULL		occurs in	NULL				Alzheimer s disease	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_6_2115_s_21	10595940	17  Because perlecan can bind to both Abeta and the amyloid precursor protein (betaPP) through its core protein or GAG moieties, 18- 21  this molecule may play a significant role in amyloid formation in Alzheimer s disease, eg, by affecting the processing of betaPP or by determining the localization of Abeta deposition at sites where perlecan is produced.	bind
56548	6	6766	6	10	NULL	0	NULL	perlecan			bind			core protein		Abeta					NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_6_2115_s_21	10595940	17  Because perlecan can bind to both Abeta and the amyloid precursor protein (betaPP) through its core protein or GAG moieties, 18- 21  this molecule may play a significant role in amyloid formation in Alzheimer s disease, eg, by affecting the processing of betaPP or by determining the localization of Abeta deposition at sites where perlecan is produced.	bind
56549	7	6766	6	10	NULL	0	NULL	perlecan			bind			core protein		betaPP					NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_6_2115_s_21	10595940	17  Because perlecan can bind to both Abeta and the amyloid precursor protein (betaPP) through its core protein or GAG moieties, 18- 21  this molecule may play a significant role in amyloid formation in Alzheimer s disease, eg, by affecting the processing of betaPP or by determining the localization of Abeta deposition at sites where perlecan is produced.	bind
56550	8	6766	6	10	NULL	0	NULL	statement 1			is an alternative to					statement 6					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2115_s_21	10595940	17  Because perlecan can bind to both Abeta and the amyloid precursor protein (betaPP) through its core protein or GAG moieties, 18- 21  this molecule may play a significant role in amyloid formation in Alzheimer s disease, eg, by affecting the processing of betaPP or by determining the localization of Abeta deposition at sites where perlecan is produced.	bind
56551	9	6766	6	10	NULL	0	NULL	statement 2			is an alternative to					statement 7					NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_6_2115_s_21	10595940	17  Because perlecan can bind to both Abeta and the amyloid precursor protein (betaPP) through its core protein or GAG moieties, 18- 21  this molecule may play a significant role in amyloid formation in Alzheimer s disease, eg, by affecting the processing of betaPP or by determining the localization of Abeta deposition at sites where perlecan is produced.	bind
57601	10	6766	6	10	NULL	0	NULL	perlecan			affects					betaPP		processing of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_6_2115_s_21	10595940	17  Because perlecan can bind to both Abeta and the amyloid precursor protein (betaPP) through its core protein or GAG moieties, 18- 21  this molecule may play a significant role in amyloid formation in Alzheimer s disease, eg, by affecting the processing of betaPP or by determining the localization of Abeta deposition at sites where perlecan is produced.	bind
23240	1	6767	5	13	NULL	NULL	NULL	FGF-2	GP		bind					tyrosine kinase receptor(s)	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_3_293_s_37	10679481	17  Binding of FGF-2 to its tyrosine kinase receptor(s) initiates a signal transduction cascade that has been shown to activate both the MAPK and PKC pathways in cardiomyocytes.	bind
23241	2	6767	5	13	NULL	NULL	NULL	statement 1	Process		initiates					signal transduction cascade	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_3_293_s_37	10679481	17  Binding of FGF-2 to its tyrosine kinase receptor(s) initiates a signal transduction cascade that has been shown to activate both the MAPK and PKC pathways in cardiomyocytes.	bind
23242	3	6767	5	13	NULL	NULL	NULL	statement 2	Process		activates					MAPK pathway	Process				NULL	in cardiomyocytes	NULL	NULL	NULL	NULL	gw60_circulationres_86_3_293_s_37	10679481	17  Binding of FGF-2 to its tyrosine kinase receptor(s) initiates a signal transduction cascade that has been shown to activate both the MAPK and PKC pathways in cardiomyocytes.	bind
23243	4	6767	5	13	NULL	NULL	NULL	statement 2	Process		activates					PKC pathway	Process				NULL	in cardiomyocytes	NULL	NULL	NULL	NULL	gw60_circulationres_86_3_293_s_37	10679481	17  Binding of FGF-2 to its tyrosine kinase receptor(s) initiates a signal transduction cascade that has been shown to activate both the MAPK and PKC pathways in cardiomyocytes.	bind
19555	1	6767	6	NULL	NULL	0	NULL	FGF-2	NULL		bind	NULL				tyrosine kinase receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_86_3_293_s_37	10679481	17  Binding of FGF-2 to its tyrosine kinase receptor(s) initiates a signal transduction cascade that has been shown to activate both the MAPK and PKC pathways in cardiomyocytes.	bind
19556	2	6767	6	NULL	NULL	0	NULL	statement 1	NULL		initiates	NULL				signal transduction cascade	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_86_3_293_s_37	10679481	17  Binding of FGF-2 to its tyrosine kinase receptor(s) initiates a signal transduction cascade that has been shown to activate both the MAPK and PKC pathways in cardiomyocytes.	bind
19557	3	6767	6	NULL	NULL	0	NULL	statement 2	NULL		activate	NULL				MAPK pathway	NULL				NULL	cardiomyocytes	0	NULL	NULL	NULL	gw60_circulationres_86_3_293_s_37	10679481	17  Binding of FGF-2 to its tyrosine kinase receptor(s) initiates a signal transduction cascade that has been shown to activate both the MAPK and PKC pathways in cardiomyocytes.	bind
19558	4	6767	6	NULL	NULL	0	NULL	statement 2	NULL		activate	NULL				PKC pathway	NULL				NULL	cardiomyocytes	0	NULL	NULL	NULL	gw60_circulationres_86_3_293_s_37	10679481	17  Binding of FGF-2 to its tyrosine kinase receptor(s) initiates a signal transduction cascade that has been shown to activate both the MAPK and PKC pathways in cardiomyocytes.	bind
19559	1	6768	6	NULL	NULL	0	NULL	hyaluronan	NULL		bind	NULL				CD44	NULL	soluble			NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_6_2159_s_74	10854236	17  Binding of hyaluronan to the soluble CD44 transfectants and their adhesion to a hyaluronan substratum were shown previously to be reduced compared to wild-type TA3/St cells and vector controls.	bind
19560	2	6768	6	NULL	NULL	0	NULL	hyaluronan	NULL		adhers to	NULL				hyaluronan substratum	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_6_2159_s_74	10854236	17  Binding of hyaluronan to the soluble CD44 transfectants and their adhesion to a hyaluronan substratum were shown previously to be reduced compared to wild-type TA3/St cells and vector controls.	bind
23256	1	6769	5	13	NULL	NULL	NULL	(LIF) receptor	GP		is					leukemia inhibitory factor receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_10_1116_s_27	10477538	17  CT-1 binds to the leukemia inhibitory factor (LIF) receptor/gp130 heterodimer and activates both mitogen-activated protein kinase and Janus kinase signal transducers and activators of transcription (STAT) signaling pathways.	bind
23257	3	6769	5	13	NULL	NULL	NULL	CT-1	GP		bind					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_10_1116_s_27	10477538	17  CT-1 binds to the leukemia inhibitory factor (LIF) receptor/gp130 heterodimer and activates both mitogen-activated protein kinase and Janus kinase signal transducers and activators of transcription (STAT) signaling pathways.	bind
23258	4	6769	5	13	NULL	NULL	NULL	statement 3	Process		activates					mitogen-activated protein kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_10_1116_s_27	10477538	17  CT-1 binds to the leukemia inhibitory factor (LIF) receptor/gp130 heterodimer and activates both mitogen-activated protein kinase and Janus kinase signal transducers and activators of transcription (STAT) signaling pathways.	bind
23259	5	6769	5	13	NULL	NULL	NULL	statement 3	Process		activates					Janus kinase signal transducers	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_10_1116_s_27	10477538	17  CT-1 binds to the leukemia inhibitory factor (LIF) receptor/gp130 heterodimer and activates both mitogen-activated protein kinase and Janus kinase signal transducers and activators of transcription (STAT) signaling pathways.	bind
23260	6	6769	5	13	NULL	NULL	NULL	CT-1	GP		activates					transcription (STAT) signaling pathways	GP	activators of 			NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_10_1116_s_27	10477538	17  CT-1 binds to the leukemia inhibitory factor (LIF) receptor/gp130 heterodimer and activates both mitogen-activated protein kinase and Janus kinase signal transducers and activators of transcription (STAT) signaling pathways.	bind
56552	2	6769	5	13	NULL	NULL	NULL	LIF receptor	GP		heterodimerize with					gp130	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_10_1116_s_27	10477538	17  CT-1 binds to the leukemia inhibitory factor (LIF) receptor/gp130 heterodimer and activates both mitogen-activated protein kinase and Janus kinase signal transducers and activators of transcription (STAT) signaling pathways.	bind
19561	1	6769	6	10	NULL	0	NULL	LIF			heterodimerize with					gp130					NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_10_1116_s_27	10477538	17  CT-1 binds to the leukemia inhibitory factor (LIF) receptor/gp130 heterodimer and activates both mitogen-activated protein kinase and Janus kinase signal transducers and activators of transcription (STAT) signaling pathways.	bind
19562	2	6769	6	NULL	NULL	0	NULL	LIF	NULL		is	NULL				leukemia inhibitory factor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_100_10_1116_s_27	10477538	17  CT-1 binds to the leukemia inhibitory factor (LIF) receptor/gp130 heterodimer and activates both mitogen-activated protein kinase and Janus kinase signal transducers and activators of transcription (STAT) signaling pathways.	bind
19563	3	6769	6	10	NULL	0	NULL	CT-1			binds to					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_10_1116_s_27	10477538	17  CT-1 binds to the leukemia inhibitory factor (LIF) receptor/gp130 heterodimer and activates both mitogen-activated protein kinase and Janus kinase signal transducers and activators of transcription (STAT) signaling pathways.	bind
19564	4	6769	6	10	NULL	0	NULL	statement 3			activates					mitogen-activated protein kinase 					NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_10_1116_s_27	10477538	17  CT-1 binds to the leukemia inhibitory factor (LIF) receptor/gp130 heterodimer and activates both mitogen-activated protein kinase and Janus kinase signal transducers and activators of transcription (STAT) signaling pathways.	bind
19565	5	6769	6	10	NULL	0	NULL	statement 3			activates					Janus kinase signal transducers					NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_10_1116_s_27	10477538	17  CT-1 binds to the leukemia inhibitory factor (LIF) receptor/gp130 heterodimer and activates both mitogen-activated protein kinase and Janus kinase signal transducers and activators of transcription (STAT) signaling pathways.	bind
56553	6	6769	6	10	NULL	0	NULL	statement 3			activates					transcription (STAT) signaling pathways		activators of 			NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_10_1116_s_27	10477538	17  CT-1 binds to the leukemia inhibitory factor (LIF) receptor/gp130 heterodimer and activates both mitogen-activated protein kinase and Janus kinase signal transducers and activators of transcription (STAT) signaling pathways.	bind
23262	1	6771	5	13	NULL	NULL	NULL	cGMP	Chemical	increased levels of	induce					calcium ion 	Chemical	decrease in;; intracellular concentration of			NULL	in platelets	NULL	NULL	NULL	NULL	gw60_circulation_97_15_1481_s_139	9576429	17  Increased cGMP levels in platelets can induce a decrease in intracellular calcium ion concentration, which may contribute to an inhibition of fibrinogen binding to the GP IIb/IIa receptor on the surface of the platelet membrane, which mediates platelet aggregation.	bind
23263	2	6771	5	13	NULL	NULL	NULL	fibrinogen	GP		bind					GP IIb/IIa receptor	GP				NULL	on the surface of the platelet membrane	NULL	NULL	NULL	NULL	gw60_circulation_97_15_1481_s_139	9576429	17  Increased cGMP levels in platelets can induce a decrease in intracellular calcium ion concentration, which may contribute to an inhibition of fibrinogen binding to the GP IIb/IIa receptor on the surface of the platelet membrane, which mediates platelet aggregation.	bind
23264	3	6771	5	13	NULL	NULL	NULL	statement 2	Process		mediate					platelets	Cell	aggregation of 			NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_15_1481_s_139	9576429	17  Increased cGMP levels in platelets can induce a decrease in intracellular calcium ion concentration, which may contribute to an inhibition of fibrinogen binding to the GP IIb/IIa receptor on the surface of the platelet membrane, which mediates platelet aggregation.	bind
23265	4	6771	5	13	NULL	NULL	NULL	statement 1	Process		contribute to		may			statement 2	Process	inhibition of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_15_1481_s_139	9576429	17  Increased cGMP levels in platelets can induce a decrease in intracellular calcium ion concentration, which may contribute to an inhibition of fibrinogen binding to the GP IIb/IIa receptor on the surface of the platelet membrane, which mediates platelet aggregation.	bind
19572	1	6771	6	NULL	NULL	0	NULL	fibrinogen	NULL		bind	NULL				GP IIb/IIa receptor	NULL				NULL	surface of the platelet membrane	0	NULL	NULL	NULL	gw60_circulation_97_15_1481_s_139	9576429	17  Increased cGMP levels in platelets can induce a decrease in intracellular calcium ion concentration, which may contribute to an inhibition of fibrinogen binding to the GP IIb/IIa receptor on the surface of the platelet membrane, which mediates platelet aggregation.	bind
19573	2	6771	6	10	NULL	0	NULL	statement 1			mediates					platelets		aggregation of 			NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_15_1481_s_139	9576429	17  Increased cGMP levels in platelets can induce a decrease in intracellular calcium ion concentration, which may contribute to an inhibition of fibrinogen binding to the GP IIb/IIa receptor on the surface of the platelet membrane, which mediates platelet aggregation.	bind
19574	3	6771	6	10	NULL	0	NULL	cGMP 		increased levels of	induce					calcium ion 		decrease in;; intracellular concentration of			NULL	platelets	NULL	NULL	NULL	NULL	gw60_circulation_97_15_1481_s_139	9576429	17  Increased cGMP levels in platelets can induce a decrease in intracellular calcium ion concentration, which may contribute to an inhibition of fibrinogen binding to the GP IIb/IIa receptor on the surface of the platelet membrane, which mediates platelet aggregation.	bind
19575	4	6771	6	10	NULL	0	NULL	statement 3			contribute to		may			statement 1		inhibition of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_15_1481_s_139	9576429	17  Increased cGMP levels in platelets can induce a decrease in intracellular calcium ion concentration, which may contribute to an inhibition of fibrinogen binding to the GP IIb/IIa receptor on the surface of the platelet membrane, which mediates platelet aggregation.	bind
28342	1	6772	5	13	NULL	NULL	NULL	B cells	Cell	sensitized	bind					HLA-DR molecules	GP	specific			NULL		NULL	NULL	NULL	NULL	gw60_circulation_98_8_786_s_143	9727549	17  Similar patterns of progressive intramolecular and intermolecular HLA-DR epitope spreading can be detected in heart transplantation recipients developing accelerated transplantation-related CAD. 18  This diversification of the immune response has been postulated to be driven by sensitized B cells that bind soluble HLA-DR molecules by using specific surface Ig receptors, endocytose these molecules, and subsequently present multiple HLA-DR allopeptides to CD4 T cells.	bind
28345	2	6772	5	13	NULL	NULL	NULL	statement 1	Process		uses					Ig receptors	GP	specific;;surface			NULL		NULL	NULL	NULL	NULL	gw60_circulation_98_8_786_s_143	9727549	17  Similar patterns of progressive intramolecular and intermolecular HLA-DR epitope spreading can be detected in heart transplantation recipients developing accelerated transplantation-related CAD. 18  This diversification of the immune response has been postulated to be driven by sensitized B cells that bind soluble HLA-DR molecules by using specific surface Ig receptors, endocytose these molecules, and subsequently present multiple HLA-DR allopeptides to CD4 T cells.	bind
28347	3	6772	5	13	NULL	NULL	NULL	statement 1	Process		undergoes					endocytosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_98_8_786_s_143	9727549	17  Similar patterns of progressive intramolecular and intermolecular HLA-DR epitope spreading can be detected in heart transplantation recipients developing accelerated transplantation-related CAD. 18  This diversification of the immune response has been postulated to be driven by sensitized B cells that bind soluble HLA-DR molecules by using specific surface Ig receptors, endocytose these molecules, and subsequently present multiple HLA-DR allopeptides to CD4 T cells.	bind
28348	4	6772	5	13	NULL	NULL	NULL	HLA-DR allopeptides	GP	multiple	is presented to		subsequently			CD4 T cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_circulation_98_8_786_s_143	9727549	17  Similar patterns of progressive intramolecular and intermolecular HLA-DR epitope spreading can be detected in heart transplantation recipients developing accelerated transplantation-related CAD. 18  This diversification of the immune response has been postulated to be driven by sensitized B cells that bind soluble HLA-DR molecules by using specific surface Ig receptors, endocytose these molecules, and subsequently present multiple HLA-DR allopeptides to CD4 T cells.	bind
19821	1	6772	6	NULL	NULL	0	NULL	B cells	NULL	sensitized	bind	NULL				HLA-DR molecules	NULL	soluble			NULL		0	NULL	NULL	NULL	gw60_circulation_98_8_786_s_143	9727549	17  Similar patterns of progressive intramolecular and intermolecular HLA-DR epitope spreading can be detected in heart transplantation recipients developing accelerated transplantation-related CAD. 18  This diversification of the immune response has been postulated to be driven by sensitized B cells that bind soluble HLA-DR molecules by using specific surface Ig receptors, endocytose these molecules, and subsequently present multiple HLA-DR allopeptides to CD4 T cells.	bind
19822	2	6772	6	10	NULL	0	NULL	statement 1			occurs by					 Ig receptors		specific;;surface			NULL		NULL	NULL	NULL	NULL	gw60_circulation_98_8_786_s_143	9727549	17  Similar patterns of progressive intramolecular and intermolecular HLA-DR epitope spreading can be detected in heart transplantation recipients developing accelerated transplantation-related CAD. 18  This diversification of the immune response has been postulated to be driven by sensitized B cells that bind soluble HLA-DR molecules by using specific surface Ig receptors, endocytose these molecules, and subsequently present multiple HLA-DR allopeptides to CD4 T cells.	bind
19823	4	6772	6	10	NULL	0	NULL	HLA-DR allopeptides			presented to					CD4 T cells					NULL		NULL	NULL	NULL	NULL	gw60_circulation_98_8_786_s_143	9727549	17  Similar patterns of progressive intramolecular and intermolecular HLA-DR epitope spreading can be detected in heart transplantation recipients developing accelerated transplantation-related CAD. 18  This diversification of the immune response has been postulated to be driven by sensitized B cells that bind soluble HLA-DR molecules by using specific surface Ig receptors, endocytose these molecules, and subsequently present multiple HLA-DR allopeptides to CD4 T cells.	bind
19824	3	6772	6	10	NULL	0	NULL	statement 1			undergoes					endocytosis					NULL		NULL	NULL	NULL	NULL	gw60_circulation_98_8_786_s_143	9727549	17  Similar patterns of progressive intramolecular and intermolecular HLA-DR epitope spreading can be detected in heart transplantation recipients developing accelerated transplantation-related CAD. 18  This diversification of the immune response has been postulated to be driven by sensitized B cells that bind soluble HLA-DR molecules by using specific surface Ig receptors, endocytose these molecules, and subsequently present multiple HLA-DR allopeptides to CD4 T cells.	bind
23266	1	6773	5	13	NULL	NULL	NULL	Raf-1	GP		bind					Ras	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_7_1159_s_116	11451745	17  The Raf-1 - bound Ras was increased by LDL exposure (see Figure 3B  ).	bind
23267	2	6773	5	13	NULL	NULL	NULL	LDL	GP	exposure	increases					Ras	GP	Raf-1 - bound			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_7_1159_s_116	11451745	17  The Raf-1 - bound Ras was increased by LDL exposure (see Figure 3B  ).	bind
19576	1	6773	6	NULL	NULL	0	NULL	Raf-1	NULL		bind	NULL				Ras	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_7_1159_s_116	11451745	17  The Raf-1 - bound Ras was increased by LDL exposure (see Figure 3B  ).	bind
19577	2	6773	6	NULL	NULL	0	NULL	statement 1	NULL		is increased by	NULL				LDL	NULL	exposure to			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_7_1159_s_116	11451745	17  The Raf-1 - bound Ras was increased by LDL exposure (see Figure 3B  ).	bind
23268	1	6774	5	13	NULL	NULL	NULL	LDL	GP		bind					PG	GP	arterial			NULL	in LNG group	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1216_s_187	9261249	17  Together these results suggest that a likely explanation for the increased binding of LDL to arterial PG in the LNG group is related to the increased apo E content.	bind
23269	2	6774	5	13	NULL	NULL	NULL	statement 1	Process	increased	is related to					apo E	GP	increased content of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1216_s_187	9261249	17  Together these results suggest that a likely explanation for the increased binding of LDL to arterial PG in the LNG group is related to the increased apo E content.	bind
19578	1	6774	6	10	NULL	0	NULL	LDL			bind					PG		arterial			NULL	LNG group	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1216_s_187	9261249	17  Together these results suggest that a likely explanation for the increased binding of LDL to arterial PG in the LNG group is related to the increased apo E content.	bind
19579	2	6774	6	10	NULL	0	NULL	statement 1			is related to					apoE 		increased content of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1216_s_187	9261249	17  Together these results suggest that a likely explanation for the increased binding of LDL to arterial PG in the LNG group is related to the increased apo E content.	bind
23271	1	6775	5	13	NULL	NULL	NULL	EC	Cell		express					growth factors	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_11_1373_s_26	16690881	17 - 19   Ang1 induces EC to express growth factors, such as endothelial-derived heparin binding EGF-like growth factor (HB-EGF) 20 and serotonin, 21 that recruit pericytes and SMC to form support for newly formed vessels.	bind
23273	2	6775	5	13	NULL	NULL	NULL	growth factors	GP		includes					HB-EGF	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_11_1373_s_26	16690881	17 - 19   Ang1 induces EC to express growth factors, such as endothelial-derived heparin binding EGF-like growth factor (HB-EGF) 20 and serotonin, 21 that recruit pericytes and SMC to form support for newly formed vessels.	bind
23274	3	6775	5	13	NULL	NULL	NULL	HB-EGF	GP		is					endothelial-derived heparin binding EGF-like growth factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_11_1373_s_26	16690881	17 - 19   Ang1 induces EC to express growth factors, such as endothelial-derived heparin binding EGF-like growth factor (HB-EGF) 20 and serotonin, 21 that recruit pericytes and SMC to form support for newly formed vessels.	bind
23275	4	6775	5	13	NULL	NULL	NULL	growth factors	GP		includes					serotonin	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_11_1373_s_26	16690881	17 - 19   Ang1 induces EC to express growth factors, such as endothelial-derived heparin binding EGF-like growth factor (HB-EGF) 20 and serotonin, 21 that recruit pericytes and SMC to form support for newly formed vessels.	bind
23276	5	6775	5	13	NULL	NULL	NULL	Ang1	GP		induces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_11_1373_s_26	16690881	17 - 19   Ang1 induces EC to express growth factors, such as endothelial-derived heparin binding EGF-like growth factor (HB-EGF) 20 and serotonin, 21 that recruit pericytes and SMC to form support for newly formed vessels.	bind
23277	6	6775	5	13	NULL	NULL	NULL	serotonin	GP		recruits					pericytes	Cell				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_11_1373_s_26	16690881	17 - 19   Ang1 induces EC to express growth factors, such as endothelial-derived heparin binding EGF-like growth factor (HB-EGF) 20 and serotonin, 21 that recruit pericytes and SMC to form support for newly formed vessels.	bind
23278	7	6775	5	13	NULL	NULL	NULL	serotonin	GP		recruits					SMC	Cell				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_11_1373_s_26	16690881	17 - 19   Ang1 induces EC to express growth factors, such as endothelial-derived heparin binding EGF-like growth factor (HB-EGF) 20 and serotonin, 21 that recruit pericytes and SMC to form support for newly formed vessels.	bind
23279	8	6775	5	13	NULL	NULL	NULL	statement 6	Process		form support for					vessels	OrganismPart	newly formed			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_11_1373_s_26	16690881	17 - 19   Ang1 induces EC to express growth factors, such as endothelial-derived heparin binding EGF-like growth factor (HB-EGF) 20 and serotonin, 21 that recruit pericytes and SMC to form support for newly formed vessels.	bind
23280	9	6775	5	13	NULL	NULL	NULL	statement 7	Process		form support for					vessels	OrganismPart	newly formed			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_11_1373_s_26	16690881	17 - 19   Ang1 induces EC to express growth factors, such as endothelial-derived heparin binding EGF-like growth factor (HB-EGF) 20 and serotonin, 21 that recruit pericytes and SMC to form support for newly formed vessels.	bind
19580	1	6775	6	NULL	NULL	0	NULL	EC	NULL		express	NULL				HB-EGF	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_11_1373_s_26	16690881	17 - 19   Ang1 induces EC to express growth factors, such as endothelial-derived heparin binding EGF-like growth factor (HB-EGF) 20 and serotonin, 21 that recruit pericytes and SMC to form support for newly formed vessels.	bind
19581	2	6775	6	NULL	NULL	0	NULL	HB-EGF	NULL		is	NULL				heparin binding EGF-like growth factor	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_11_1373_s_26	16690881	17 - 19   Ang1 induces EC to express growth factors, such as endothelial-derived heparin binding EGF-like growth factor (HB-EGF) 20 and serotonin, 21 that recruit pericytes and SMC to form support for newly formed vessels.	bind
19582	3	6775	6	NULL	NULL	0	NULL	Ang1	NULL		induces	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_11_1373_s_26	16690881	17 - 19   Ang1 induces EC to express growth factors, such as endothelial-derived heparin binding EGF-like growth factor (HB-EGF) 20 and serotonin, 21 that recruit pericytes and SMC to form support for newly formed vessels.	bind
19583	6	6775	6	10	NULL	0	NULL	statement 4			form support for					 vessels		newly formed			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_11_1373_s_26	16690881	17 - 19   Ang1 induces EC to express growth factors, such as endothelial-derived heparin binding EGF-like growth factor (HB-EGF) 20 and serotonin, 21 that recruit pericytes and SMC to form support for newly formed vessels.	bind
19584	7	6775	6	10	NULL	0	NULL	statement 5			forms support for					 vessels		newly formed			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_11_1373_s_26	16690881	17 - 19   Ang1 induces EC to express growth factors, such as endothelial-derived heparin binding EGF-like growth factor (HB-EGF) 20 and serotonin, 21 that recruit pericytes and SMC to form support for newly formed vessels.	bind
19585	4	6775	6	10	NULL	0	NULL	serotonin			recruit					pericytes					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_11_1373_s_26	16690881	17 - 19   Ang1 induces EC to express growth factors, such as endothelial-derived heparin binding EGF-like growth factor (HB-EGF) 20 and serotonin, 21 that recruit pericytes and SMC to form support for newly formed vessels.	bind
19586	5	6775	6	10	NULL	0	NULL	serotonin			recruit					SMC					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_11_1373_s_26	16690881	17 - 19   Ang1 induces EC to express growth factors, such as endothelial-derived heparin binding EGF-like growth factor (HB-EGF) 20 and serotonin, 21 that recruit pericytes and SMC to form support for newly formed vessels.	bind
56554	8	6775	6	10	NULL	0	NULL	HB-EGF			is a type of					growth factor					NULL		0	NULL	NULL	NULL	gw70_circulationres_98_11_1373_s_26	16690881	17 - 19   Ang1 induces EC to express growth factors, such as endothelial-derived heparin binding EGF-like growth factor (HB-EGF) 20 and serotonin, 21 that recruit pericytes and SMC to form support for newly formed vessels.	bind
56555	9	6775	6	10	NULL	0	NULL	serotonin			is a type of					growth factor					NULL		0	NULL	NULL	NULL	gw70_circulationres_98_11_1373_s_26	16690881	17 - 19   Ang1 induces EC to express growth factors, such as endothelial-derived heparin binding EGF-like growth factor (HB-EGF) 20 and serotonin, 21 that recruit pericytes and SMC to form support for newly formed vessels.	bind
23283	1	6776	5	13	NULL	NULL	NULL	myocardial ischemia	MedicalFinding		leads to					Mgi	Chemical	increase in			NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_3_975_s_36	9264509	17 18  During myocardial ischemia, Mgi increases with degradation of ATP, which binds most Mgi. 19 20 21 22  Increased Mgi levels could be harmful to cardiac cells if they are compensated for by Mg2+ efflux through Na+-Mg2+ countertransport, which in turn would promote excess cellular Ca2+ gain through Na+-Ca2+ exchange.	bind
23284	2	6776	5	13	NULL	NULL	NULL	statement 1	Process		occurs with					ATP	Chemical	degradation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_3_975_s_36	9264509	17 18  During myocardial ischemia, Mgi increases with degradation of ATP, which binds most Mgi. 19 20 21 22  Increased Mgi levels could be harmful to cardiac cells if they are compensated for by Mg2+ efflux through Na+-Mg2+ countertransport, which in turn would promote excess cellular Ca2+ gain through Na+-Ca2+ exchange.	bind
23285	3	6776	5	13	NULL	NULL	NULL	ATP	Chemical		bind					Mgi	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_3_975_s_36	9264509	17 18  During myocardial ischemia, Mgi increases with degradation of ATP, which binds most Mgi. 19 20 21 22  Increased Mgi levels could be harmful to cardiac cells if they are compensated for by Mg2+ efflux through Na+-Mg2+ countertransport, which in turn would promote excess cellular Ca2+ gain through Na+-Ca2+ exchange.	bind
23286	4	6776	5	13	NULL	NULL	NULL	Mgi	Chemical	increased levels of	is harmful for		could be			cardiac cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_3_975_s_36	9264509	17 18  During myocardial ischemia, Mgi increases with degradation of ATP, which binds most Mgi. 19 20 21 22  Increased Mgi levels could be harmful to cardiac cells if they are compensated for by Mg2+ efflux through Na+-Mg2+ countertransport, which in turn would promote excess cellular Ca2+ gain through Na+-Ca2+ exchange.	bind
23287	5	6776	5	13	NULL	NULL	NULL	statement 4	Process		occurs when					Mg2+ 	Chemical	compensated for by efflux of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_3_975_s_36	9264509	17 18  During myocardial ischemia, Mgi increases with degradation of ATP, which binds most Mgi. 19 20 21 22  Increased Mgi levels could be harmful to cardiac cells if they are compensated for by Mg2+ efflux through Na+-Mg2+ countertransport, which in turn would promote excess cellular Ca2+ gain through Na+-Ca2+ exchange.	bind
23288	6	6776	5	13	NULL	NULL	NULL	Mg2+ efflux	Process		occurs through					Na+-Mg2+ 	Process	countertransport of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_3_975_s_36	9264509	17 18  During myocardial ischemia, Mgi increases with degradation of ATP, which binds most Mgi. 19 20 21 22  Increased Mgi levels could be harmful to cardiac cells if they are compensated for by Mg2+ efflux through Na+-Mg2+ countertransport, which in turn would promote excess cellular Ca2+ gain through Na+-Ca2+ exchange.	bind
23289	7	6776	5	13	NULL	NULL	NULL	statement 5	Process		promotes					Ca2+	Chemical	excess cellular gain of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_3_975_s_36	9264509	17 18  During myocardial ischemia, Mgi increases with degradation of ATP, which binds most Mgi. 19 20 21 22  Increased Mgi levels could be harmful to cardiac cells if they are compensated for by Mg2+ efflux through Na+-Mg2+ countertransport, which in turn would promote excess cellular Ca2+ gain through Na+-Ca2+ exchange.	bind
23291	8	6776	5	13	NULL	NULL	NULL	statement 7	Process		occurs through					Na+-Ca2+ 	Chemical	exchange of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_3_975_s_36	9264509	17 18  During myocardial ischemia, Mgi increases with degradation of ATP, which binds most Mgi. 19 20 21 22  Increased Mgi levels could be harmful to cardiac cells if they are compensated for by Mg2+ efflux through Na+-Mg2+ countertransport, which in turn would promote excess cellular Ca2+ gain through Na+-Ca2+ exchange.	bind
19825	1	6776	6	NULL	NULL	0	NULL	Mgi	NULL		increases with	NULL				ATP	NULL	degradation of			NULL		0	NULL	NULL	NULL	gw60_circulation_96_3_975_s_36	9264509	17 18  During myocardial ischemia, Mgi increases with degradation of ATP, which binds most Mgi. 19 20 21 22  Increased Mgi levels could be harmful to cardiac cells if they are compensated for by Mg2+ efflux through Na+-Mg2+ countertransport, which in turn would promote excess cellular Ca2+ gain through Na+-Ca2+ exchange.	bind
19826	2	6776	6	NULL	NULL	0	NULL	statement 1	NULL		occurs during	NULL				myocardial ischemia	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_96_3_975_s_36	9264509	17 18  During myocardial ischemia, Mgi increases with degradation of ATP, which binds most Mgi. 19 20 21 22  Increased Mgi levels could be harmful to cardiac cells if they are compensated for by Mg2+ efflux through Na+-Mg2+ countertransport, which in turn would promote excess cellular Ca2+ gain through Na+-Ca2+ exchange.	bind
20098	3	6776	6	NULL	NULL	0	NULL	Mgi	NULL		bind	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_96_3_975_s_36	9264509	17 18  During myocardial ischemia, Mgi increases with degradation of ATP, which binds most Mgi. 19 20 21 22  Increased Mgi levels could be harmful to cardiac cells if they are compensated for by Mg2+ efflux through Na+-Mg2+ countertransport, which in turn would promote excess cellular Ca2+ gain through Na+-Ca2+ exchange.	bind
56556	4	6776	6	10	NULL	0	NULL	Mgi 		increased levels of	harmful for		could be			cardiac cells					NULL		0	NULL	NULL	NULL	gw60_circulation_96_3_975_s_36	9264509	17 18  During myocardial ischemia, Mgi increases with degradation of ATP, which binds most Mgi. 19 20 21 22  Increased Mgi levels could be harmful to cardiac cells if they are compensated for by Mg2+ efflux through Na+-Mg2+ countertransport, which in turn would promote excess cellular Ca2+ gain through Na+-Ca2+ exchange.	bind
56557	5	6776	6	10	NULL	0	NULL	statement 4			occurs when					Mg2+		compensated for by efflux of			NULL		0	NULL	NULL	NULL	gw60_circulation_96_3_975_s_36	9264509	17 18  During myocardial ischemia, Mgi increases with degradation of ATP, which binds most Mgi. 19 20 21 22  Increased Mgi levels could be harmful to cardiac cells if they are compensated for by Mg2+ efflux through Na+-Mg2+ countertransport, which in turn would promote excess cellular Ca2+ gain through Na+-Ca2+ exchange.	bind
56558	6	6776	6	10	NULL	0	NULL	Mg2+		efflux of	occur through					Na+-Mg2+ 		countertransport of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_3_975_s_36	9264509	17 18  During myocardial ischemia, Mgi increases with degradation of ATP, which binds most Mgi. 19 20 21 22  Increased Mgi levels could be harmful to cardiac cells if they are compensated for by Mg2+ efflux through Na+-Mg2+ countertransport, which in turn would promote excess cellular Ca2+ gain through Na+-Ca2+ exchange.	bind
56559	7	6776	6	10	NULL	0	NULL	statement 5			promotes					Ca2+		excess cellular gain of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_3_975_s_36	9264509	17 18  During myocardial ischemia, Mgi increases with degradation of ATP, which binds most Mgi. 19 20 21 22  Increased Mgi levels could be harmful to cardiac cells if they are compensated for by Mg2+ efflux through Na+-Mg2+ countertransport, which in turn would promote excess cellular Ca2+ gain through Na+-Ca2+ exchange.	bind
56560	8	6776	6	10	NULL	0	NULL	statement 7			occur through					Na+-Ca2+		exchange of			NULL		0	NULL	NULL	NULL	gw60_circulation_96_3_975_s_36	9264509	17 18  During myocardial ischemia, Mgi increases with degradation of ATP, which binds most Mgi. 19 20 21 22  Increased Mgi levels could be harmful to cardiac cells if they are compensated for by Mg2+ efflux through Na+-Mg2+ countertransport, which in turn would promote excess cellular Ca2+ gain through Na+-Ca2+ exchange.	bind
23292	1	6777	5	13	NULL	NULL	NULL	NOS1	GP		bind			latch domain		calmodulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_3_363_s_15	8781470	17 18  In NOS1 and NOS3, physiological concentrations of Ca2+ in cells regulate the binding of calmodulin to the "`latch domain,"` thereby initiating electron transfer from the flavins to the heme moieties.	bind
23293	2	6777	5	13	NULL	NULL	NULL	NOS3	GP		bind			latch domain		calmodulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_3_363_s_15	8781470	17 18  In NOS1 and NOS3, physiological concentrations of Ca2+ in cells regulate the binding of calmodulin to the "`latch domain,"` thereby initiating electron transfer from the flavins to the heme moieties.	bind
23294	3	6777	5	13	NULL	NULL	NULL	Ca2+	Chemical	physiological concentrations of	regulates					statement 1	Process				NULL	in cells	NULL	NULL	NULL	NULL	gw60_circulationres_79_3_363_s_15	8781470	17 18  In NOS1 and NOS3, physiological concentrations of Ca2+ in cells regulate the binding of calmodulin to the "`latch domain,"` thereby initiating electron transfer from the flavins to the heme moieties.	bind
23297	4	6777	5	13	NULL	NULL	NULL	ca2+	Chemical	physiological concentrations of	regulates					statement 2	Process				NULL	in cells	NULL	NULL	NULL	NULL	gw60_circulationres_79_3_363_s_15	8781470	17 18  In NOS1 and NOS3, physiological concentrations of Ca2+ in cells regulate the binding of calmodulin to the "`latch domain,"` thereby initiating electron transfer from the flavins to the heme moieties.	bind
23298	5	6777	5	13	NULL	NULL	NULL	flavins	Chemical	electrons from	transferred to					heme moieties	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_3_363_s_15	8781470	17 18  In NOS1 and NOS3, physiological concentrations of Ca2+ in cells regulate the binding of calmodulin to the "`latch domain,"` thereby initiating electron transfer from the flavins to the heme moieties.	bind
23299	6	6777	5	13	NULL	NULL	NULL	statement 3	Process		initiates					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_3_363_s_15	8781470	17 18  In NOS1 and NOS3, physiological concentrations of Ca2+ in cells regulate the binding of calmodulin to the "`latch domain,"` thereby initiating electron transfer from the flavins to the heme moieties.	bind
56561	7	6777	5	13	NULL	NULL	NULL	statement 4	Process		initiates					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_3_363_s_15	8781470	17 18  In NOS1 and NOS3, physiological concentrations of Ca2+ in cells regulate the binding of calmodulin to the "`latch domain,"` thereby initiating electron transfer from the flavins to the heme moieties.	bind
19587	1	6777	6	10	NULL	0	NULL	calmodulin			bind					NOS1			latch domain		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_3_363_s_15	8781470	17 18  In NOS1 and NOS3, physiological concentrations of Ca2+ in cells regulate the binding of calmodulin to the "`latch domain,"` thereby initiating electron transfer from the flavins to the heme moieties.	bind
19588	2	6777	6	10	NULL	0	NULL	Calmodulin			bind					NOS3			latch domain		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_3_363_s_15	8781470	17 18  In NOS1 and NOS3, physiological concentrations of Ca2+ in cells regulate the binding of calmodulin to the "`latch domain,"` thereby initiating electron transfer from the flavins to the heme moieties.	bind
19589	3	6777	6	NULL	NULL	0	NULL	Ca2+	NULL	physiological concentrations of	regulates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_79_3_363_s_15	8781470	17 18  In NOS1 and NOS3, physiological concentrations of Ca2+ in cells regulate the binding of calmodulin to the "`latch domain,"` thereby initiating electron transfer from the flavins to the heme moieties.	bind
19590	4	6777	6	NULL	NULL	0	NULL	Ca2+	NULL	physiological concentrations of	regulates	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_79_3_363_s_15	8781470	17 18  In NOS1 and NOS3, physiological concentrations of Ca2+ in cells regulate the binding of calmodulin to the "`latch domain,"` thereby initiating electron transfer from the flavins to the heme moieties.	bind
19591	5	6777	6	10	NULL	0	NULL	flavins		electron from	transferred to					heme moieties					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_3_363_s_15	8781470	17 18  In NOS1 and NOS3, physiological concentrations of Ca2+ in cells regulate the binding of calmodulin to the "`latch domain,"` thereby initiating electron transfer from the flavins to the heme moieties.	bind
19592	6	6777	6	10	NULL	0	NULL	statement 3			initiates					statement 5					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_3_363_s_15	8781470	17 18  In NOS1 and NOS3, physiological concentrations of Ca2+ in cells regulate the binding of calmodulin to the "`latch domain,"` thereby initiating electron transfer from the flavins to the heme moieties.	bind
19593	7	6777	6	10	NULL	0	NULL	statement 4			initiates					statement 5					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_3_363_s_15	8781470	17 18  In NOS1 and NOS3, physiological concentrations of Ca2+ in cells regulate the binding of calmodulin to the "`latch domain,"` thereby initiating electron transfer from the flavins to the heme moieties.	bind
23319	1	6778	5	13	NULL	NULL	NULL	osteopontin	GP		regulate		may			vascular calcification	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_2_166_s_37	9933248	17 18 19  These data suggest that osteopontin might be an important regulator of vascular calcification.	bind
19594	1	6778	6	NULL	NULL	0	NULL	osteopontin	NULL		regulates	NULL	may			vascular calcification	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_2_166_s_37	9933248	17 18 19  These data suggest that osteopontin might be an important regulator of vascular calcification.	bind
23321	1	6779	5	13	NULL	NULL	NULL	E1A gene product	GP	adenovirus	bind					RB	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_7_820_s_184	10205150	17 18 29 47 48 49  The adenovirus E1A gene product binds to RB, which releases E2F, and E1A-induced apoptosis is dependent on E2F.	bind
23322	2	6779	5	13	NULL	NULL	NULL	RB	GP		release					E2F	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_7_820_s_184	10205150	17 18 29 47 48 49  The adenovirus E1A gene product binds to RB, which releases E2F, and E1A-induced apoptosis is dependent on E2F.	bind
23324	4	6779	5	13	NULL	NULL	NULL	statement 3	Process		is dependent on					E2F	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_7_820_s_184	10205150	17 18 29 47 48 49  The adenovirus E1A gene product binds to RB, which releases E2F, and E1A-induced apoptosis is dependent on E2F.	bind
44689	3	6779	5	13	NULL	NULL	NULL	E1A	GP		induce					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_7_820_s_184	10205150	17 18 29 47 48 49  The adenovirus E1A gene product binds to RB, which releases E2F, and E1A-induced apoptosis is dependent on E2F.	bind
19595	1	6779	6	NULL	NULL	0	NULL	E1A gene product	NULL	Adenovirus	bind	NULL				RB	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_7_820_s_184	10205150	17 18 29 47 48 49  The adenovirus E1A gene product binds to RB, which releases E2F, and E1A-induced apoptosis is dependent on E2F.	bind
19596	2	6779	6	NULL	NULL	0	NULL	RB	NULL		releases	NULL				E2F	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_7_820_s_184	10205150	17 18 29 47 48 49  The adenovirus E1A gene product binds to RB, which releases E2F, and E1A-induced apoptosis is dependent on E2F.	bind
19597	4	6779	6	10	NULL	0	NULL	statement 3	NULL		is dependent on	NULL				E2F	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_7_820_s_184	10205150	17 18 29 47 48 49  The adenovirus E1A gene product binds to RB, which releases E2F, and E1A-induced apoptosis is dependent on E2F.	bind
44690	3	6779	6	10	NULL	0	NULL	E1A	NULL		induce	NULL				apoptosis	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_7_820_s_184	10205150	17 18 29 47 48 49  The adenovirus E1A gene product binds to RB, which releases E2F, and E1A-induced apoptosis is dependent on E2F.	bind
23326	1	6780	5	13	NULL	NULL	NULL	FVII 	GP		bind					TG-rich particles	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_8_1539_s_122	9301633	17 21  The correlation between FVIIc and lipoproteins may be explained by the binding of FVII to TG-rich particles.	bind
19598	1	6780	6	NULL	NULL	0	NULL	FVII	NULL		bind	NULL				TG-rich particles	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_8_1539_s_122	9301633	17 21  The correlation between FVIIc and lipoproteins may be explained by the binding of FVII to TG-rich particles.	bind
28356	1	6781	5	13	NULL	NULL	NULL	apolipoprotein	GP		mediate					lipid efflux	Process	defect in			NULL	in Tangier cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1813_s_181	9327782	17 27 38 39  The lack of acceptor specificity in the apolipoprotein-mediated lipid efflux defect in Tangier cells makes it less likely that a defect in the binding of apoA-I to Tangier cells 11  is the mechanism for the decreased lipid efflux.	bind
28358	2	6781	5	13	NULL	NULL	NULL	acceptor specificity	Process		is absent in					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1813_s_181	9327782	17 27 38 39  The lack of acceptor specificity in the apolipoprotein-mediated lipid efflux defect in Tangier cells makes it less likely that a defect in the binding of apoA-I to Tangier cells 11  is the mechanism for the decreased lipid efflux.	bind
28359	3	6781	5	13	NULL	NULL	NULL	apoA-I	GP		bind					Tangier cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1813_s_181	9327782	17 27 38 39  The lack of acceptor specificity in the apolipoprotein-mediated lipid efflux defect in Tangier cells makes it less likely that a defect in the binding of apoA-I to Tangier cells 11  is the mechanism for the decreased lipid efflux.	bind
28362	4	6781	5	13	NULL	NULL	NULL	statement 3	Process	defect in	decreases					lipid efflux	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1813_s_181	9327782	17 27 38 39  The lack of acceptor specificity in the apolipoprotein-mediated lipid efflux defect in Tangier cells makes it less likely that a defect in the binding of apoA-I to Tangier cells 11  is the mechanism for the decreased lipid efflux.	bind
19599	1	6781	6	NULL	NULL	0	NULL	apoA-I	NULL		bind	NULL				Tangier cells	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1813_s_181	9327782	17 27 38 39  The lack of acceptor specificity in the apolipoprotein-mediated lipid efflux defect in Tangier cells makes it less likely that a defect in the binding of apoA-I to Tangier cells 11  is the mechanism for the decreased lipid efflux.	bind
19600	3	6781	6	10	NULL	0	NULL	acceptor specificity	NULL		lacks in	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1813_s_181	9327782	17 27 38 39  The lack of acceptor specificity in the apolipoprotein-mediated lipid efflux defect in Tangier cells makes it less likely that a defect in the binding of apoA-I to Tangier cells 11  is the mechanism for the decreased lipid efflux.	bind
44692	2	6781	6	10	NULL	0	NULL	apolipoprotein	NULL		mediates	NULL				lipid efflux	NULL	defect in			NULL	Tangier cells	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1813_s_181	9327782	17 27 38 39  The lack of acceptor specificity in the apolipoprotein-mediated lipid efflux defect in Tangier cells makes it less likely that a defect in the binding of apoA-I to Tangier cells 11  is the mechanism for the decreased lipid efflux.	bind
44693	4	6781	6	10	NULL	0	NULL	statement 1	NULL	defect in	decrease	NULL				lipid efflux	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1813_s_181	9327782	17 27 38 39  The lack of acceptor specificity in the apolipoprotein-mediated lipid efflux defect in Tangier cells makes it less likely that a defect in the binding of apoA-I to Tangier cells 11  is the mechanism for the decreased lipid efflux.	bind
23328	1	6782	5	13	NULL	NULL	NULL	nuclear protein	GP		bind					NF-kappaB-3'	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_3_295_s_266	9710122	17 34  35  Our results have shown that HMG I(Y) protein facilitates nuclear protein binding with NF-kappaB-3' and with TATA box elements.	bind
23329	2	6782	5	13	NULL	NULL	NULL	HMG I(Y) protein	GP		facilitates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_3_295_s_266	9710122	17 34  35  Our results have shown that HMG I(Y) protein facilitates nuclear protein binding with NF-kappaB-3' and with TATA box elements.	bind
23330	3	6782	5	13	NULL	NULL	NULL	nuclear protein	GP		bind									TATA box elements	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_3_295_s_266	9710122	17 34  35  Our results have shown that HMG I(Y) protein facilitates nuclear protein binding with NF-kappaB-3' and with TATA box elements.	bind
23331	4	6782	5	13	NULL	NULL	NULL	HMG I(Y) protein	GP		facilitates					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_3_295_s_266	9710122	17 34  35  Our results have shown that HMG I(Y) protein facilitates nuclear protein binding with NF-kappaB-3' and with TATA box elements.	bind
19827	1	6782	6	NULL	NULL	0	NULL	nuclear protein	NULL		bind	NULL					NULL			NF-kappaB-3' element	NULL		0	NULL	NULL	NULL	gw60_circulationres_83_3_295_s_266	9710122	17 34  35  Our results have shown that HMG I(Y) protein facilitates nuclear protein binding with NF-kappaB-3' and with TATA box elements.	bind
19828	2	6782	6	NULL	NULL	0	NULL	Nuclear protein	NULL		bind	NULL					NULL			TATA box	NULL		0	NULL	NULL	NULL	gw60_circulationres_83_3_295_s_266	9710122	17 34  35  Our results have shown that HMG I(Y) protein facilitates nuclear protein binding with NF-kappaB-3' and with TATA box elements.	bind
19829	3	6782	6	NULL	NULL	0	NULL	HMG I(Y) protein	NULL		facilitates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_3_295_s_266	9710122	17 34  35  Our results have shown that HMG I(Y) protein facilitates nuclear protein binding with NF-kappaB-3' and with TATA box elements.	bind
19830	4	6782	6	NULL	NULL	0	NULL	HMG I(Y) protein	NULL		facilitates	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_3_295_s_266	9710122	17 34  35  Our results have shown that HMG I(Y) protein facilitates nuclear protein binding with NF-kappaB-3' and with TATA box elements.	bind
23332	1	6783	5	13	NULL	NULL	NULL	Atorvastatin	Chemical		inhibit					ethinyl estradiol	Chemical	metabolism of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_1_32_s_112	12515739	17 Atorvastatin has previously been shown to inhibit the metabolism of only a few substrates, such as ethinyl estradiol, 19 which binds CYP3A4  30-fold less tightly than atorvastatin lactone and is also present in vivo at low concentrations.	bind
23333	2	6783	5	13	NULL	NULL	NULL	ethinyl estradiol	Chemical		bind					CYP3A4	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_1_32_s_112	12515739	17 Atorvastatin has previously been shown to inhibit the metabolism of only a few substrates, such as ethinyl estradiol, 19 which binds CYP3A4  30-fold less tightly than atorvastatin lactone and is also present in vivo at low concentrations.	bind
23334	3	6783	5	13	NULL	NULL	NULL	ethinyl estradiol	Chemical		bind					atorvastatin lactone	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_1_32_s_112	12515739	17 Atorvastatin has previously been shown to inhibit the metabolism of only a few substrates, such as ethinyl estradiol, 19 which binds CYP3A4  30-fold less tightly than atorvastatin lactone and is also present in vivo at low concentrations.	bind
23335	4	6783	5	13	NULL	NULL	NULL	statement 2	Process		less tightly than					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_1_32_s_112	12515739	17 Atorvastatin has previously been shown to inhibit the metabolism of only a few substrates, such as ethinyl estradiol, 19 which binds CYP3A4  30-fold less tightly than atorvastatin lactone and is also present in vivo at low concentrations.	bind
19602	1	6783	6	NULL	NULL	0	NULL	ethinyl estradiol	NULL		bind	NULL				CYP3A4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_107_1_32_s_112	12515739	17 Atorvastatin has previously been shown to inhibit the metabolism of only a few substrates, such as ethinyl estradiol, 19 which binds CYP3A4  30-fold less tightly than atorvastatin lactone and is also present in vivo at low concentrations.	bind
19603	2	6783	6	NULL	NULL	0	NULL	atorvastatin lactone	NULL		bind	NULL				CYP3A4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_107_1_32_s_112	12515739	17 Atorvastatin has previously been shown to inhibit the metabolism of only a few substrates, such as ethinyl estradiol, 19 which binds CYP3A4  30-fold less tightly than atorvastatin lactone and is also present in vivo at low concentrations.	bind
19604	3	6783	6	NULL	NULL	0	NULL	statement 2	NULL		is less as compared to	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_107_1_32_s_112	12515739	17 Atorvastatin has previously been shown to inhibit the metabolism of only a few substrates, such as ethinyl estradiol, 19 which binds CYP3A4  30-fold less tightly than atorvastatin lactone and is also present in vivo at low concentrations.	bind
19605	4	6783	6	NULL	NULL	0	NULL	Atorvastatin	NULL		inhibits	NULL				ethinyl estradiol	NULL	metabolism of 			NULL		0	NULL	NULL	NULL	gw60_circulation_107_1_32_s_112	12515739	17 Atorvastatin has previously been shown to inhibit the metabolism of only a few substrates, such as ethinyl estradiol, 19 which binds CYP3A4  30-fold less tightly than atorvastatin lactone and is also present in vivo at low concentrations.	bind
23390	1	6784	5	13	NULL	NULL	NULL	CD40L	GP		bind					CD40 receptor	GP				NULL	on the surface of endothelial cells	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23391	2	6784	5	13	NULL	NULL	NULL	CD40L	GP		bind					CD40 receptor	GP				NULL	on the surface of smooth muscle cells	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23392	3	6784	5	13	NULL	NULL	NULL	CD40L	GP		bind					CD40 receptor	GP				NULL	on the surface of macrophages	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23393	4	6784	5	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23394	5	6784	5	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23395	6	6784	5	13	NULL	NULL	NULL	statement 1	Process		triggers					cytokines	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23396	7	6784	5	13	NULL	NULL	NULL	statement 1	Process		triggers					chemokines	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23397	8	6784	5	13	NULL	NULL	NULL	statement 1	Process		triggers					growth factors	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23398	9	6784	5	13	NULL	NULL	NULL	statement 1	Process		triggers					matrix metalloproteinases	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23399	10	6784	5	13	NULL	NULL	NULL	statement 1	Process		triggers					adhesion molecules	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23400	11	6784	5	13	NULL	NULL	NULL	statement 1	Process		triggers					procoagulants	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23401	12	6784	5	13	NULL	NULL	NULL	statement 2	Process		triggers					cytokines	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23402	13	6784	5	13	NULL	NULL	NULL	statement 2	Process		triggers					chemokines	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23403	14	6784	5	13	NULL	NULL	NULL	statement 2	Process		triggers					growth factors	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23404	15	6784	5	13	NULL	NULL	NULL	statement 2	Process		triggers					matrix metalloproteinases	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23405	16	6784	5	13	NULL	NULL	NULL	statement 2	Process		triggers					adhesion molecules	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23406	17	6784	5	13	NULL	NULL	NULL	statement 2	Process		triggers					procoagulants	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23407	18	6784	5	13	NULL	NULL	NULL	statement 3	Process		triggers					cytokines	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23408	19	6784	5	13	NULL	NULL	NULL	statement 3	Process		triggers					chemokines	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23409	20	6784	5	13	NULL	NULL	NULL	statement 3	Process		triggers					growth factors	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23410	21	6784	5	13	NULL	NULL	NULL	statement 3	Process		triggers					matrix metalloproteinases	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23411	22	6784	5	13	NULL	NULL	NULL	statement 3	Process		triggers					adhesion molecules	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23412	23	6784	5	13	NULL	NULL	NULL	statement 3	Process		triggers					procoagulants	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23413	24	6784	5	13	NULL	NULL	NULL	statement 6	Process		elaborate					inflammatory response	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23414	25	6784	5	13	NULL	NULL	NULL	statement 7	Process		elaborate					inflammatory response	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23415	26	6784	5	13	NULL	NULL	NULL	statement 8	Process		elaborate					inflammatory response	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23416	27	6784	5	13	NULL	NULL	NULL	statement 9	Process		elaborate					inflammatory response	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23417	28	6784	5	13	NULL	NULL	NULL	statement 10	Process		elaborate					inflammatory response	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23418	29	6784	5	13	NULL	NULL	NULL	statement 11	Process		elaborate					inflammatory response	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23419	30	6784	5	13	NULL	NULL	NULL	statement 12	Process		elaborate					inflammatory response	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23420	31	6784	5	13	NULL	NULL	NULL	statement 13	Process		elaborate					inflammatory response	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23421	32	6784	5	13	NULL	NULL	NULL	statement 14	Process		elaborate					inflammatory response	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23422	33	6784	5	13	NULL	NULL	NULL	statement 15	Process		elaborate					inflammatory response	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23423	34	6784	5	13	NULL	NULL	NULL	statement 16	Process		elaborate					inflammatory response	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23424	35	6784	5	13	NULL	NULL	NULL	statement 17	Process		elaborate					inflammatory response	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23425	36	6784	5	13	NULL	NULL	NULL	statement 18	Process		elaborate					inflammatory response	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23426	37	6784	5	13	NULL	NULL	NULL	statement 19	Process		elaborate					inflammatory response	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23427	38	6784	5	13	NULL	NULL	NULL	statement 20	Process		elaborate					inflammatory response	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23428	39	6784	5	13	NULL	NULL	NULL	statement 21	Process		elaborate					inflammatory response	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23429	40	6784	5	13	NULL	NULL	NULL	statement 22	Process		elaborate					inflammatory response	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23430	41	6784	5	13	NULL	NULL	NULL	statement 23	Process		elaborate					inflammatory response	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
19606	1	6784	6	NULL	NULL	0	NULL	CD40L	NULL		bind	NULL				CD40 receptor	NULL				NULL	surface of endothelial cells	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
19669	2	6784	6	NULL	NULL	0	NULL	CD40L	NULL		bind	NULL				CD40 receptor	NULL				NULL	surface of smooth muscle cells	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
19670	3	6784	6	NULL	NULL	0	NULL	CD40L	NULL		bind	NULL				CD40 receptor	NULL				NULL	surface of macrophages	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
19671	4	6784	6	NULL	NULL	0	NULL	statement 1	NULL		triggers	NULL				cytokines	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
20099	5	6784	6	NULL	NULL	0	NULL	statement 2	NULL		triggers	NULL				cytokines	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
20100	6	6784	6	NULL	NULL	0	NULL	statement 3	NULL		triggers	NULL				cytokines	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
20101	7	6784	6	NULL	NULL	0	NULL	statement 1	NULL		triggers	NULL				chemokines	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
20102	8	6784	6	NULL	NULL	0	NULL	statement 2	NULL		triggers	NULL				chemokines	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
20103	9	6784	6	NULL	NULL	0	NULL	statement 3	NULL		triggers	NULL				chemokines	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
20104	10	6784	6	NULL	NULL	0	NULL	statement 1	NULL		triggers	NULL				growth factors	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
20105	11	6784	6	NULL	NULL	0	NULL	statement 2	NULL		triggers	NULL				growth factors	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
20106	12	6784	6	NULL	NULL	0	NULL	statement 3	NULL		triggers	NULL				growth factors	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
20107	13	6784	6	NULL	NULL	0	NULL	statement 1	NULL		triggers	NULL				matrix metalloproteinases	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
20108	14	6784	6	NULL	NULL	0	NULL	statement 2	NULL		triggers	NULL				matrix metalloproteinases	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
20109	15	6784	6	NULL	NULL	0	NULL	statement 3	NULL		triggers	NULL				matrix metalloproteinases	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
20110	16	6784	6	NULL	NULL	0	NULL	statement 1	NULL		triggers	NULL				adhesion molecules	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
20111	17	6784	6	NULL	NULL	0	NULL	statement 2	NULL		triggers	NULL				adhesion molecules	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
20112	18	6784	6	NULL	NULL	0	NULL	statement 3	NULL		triggers	NULL				adhesion molecules	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
20113	19	6784	6	NULL	NULL	0	NULL	statement 1	NULL		triggers	NULL				procoagulants	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
20114	20	6784	6	NULL	NULL	0	NULL	statement 2	NULL		triggers	NULL				procoagulants	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
20115	21	6784	6	NULL	NULL	0	NULL	statement 3	NULL		triggers	NULL				procoagulants	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1088_s_20	15923539	17 Binding of CD40L to the CD40 receptor on the surface of endothelial cells, smooth muscle cells, or macrophages triggers the expression of cytokines, chemokines, growth factors, matrix metalloproteinases, adhesion molecules, and procoagulants, all of which elaborate the inflammatory response.	bind
23432	1	6785	5	13	NULL	NULL	NULL	self-associative interaction	Process		influence					ROCKs	GP	kinase activity of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_322_s_48	16484628	17 In addition to this self-associative interaction, oligomerization (dimerization) also influences the kinase activity of ROCKs by regulating its affinity for ATP. 18 Binding of active GTP-bound form of RhoA to RBD stimulates the phosphotransferase activity of ROCKs by disrupting the interaction between the catalytic and the inhibitory C-terminal region of the enzyme ( Figure 2).	bind
23433	2	6785	5	13	NULL	NULL	NULL	oligomerization (dimerization)	Process		influence					ROCKs	GP	kinase activity of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_322_s_48	16484628	17 In addition to this self-associative interaction, oligomerization (dimerization) also influences the kinase activity of ROCKs by regulating its affinity for ATP. 18 Binding of active GTP-bound form of RhoA to RBD stimulates the phosphotransferase activity of ROCKs by disrupting the interaction between the catalytic and the inhibitory C-terminal region of the enzyme ( Figure 2).	bind
23434	3	6785	5	13	NULL	NULL	NULL	ROCKs	GP		has affinity for					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_322_s_48	16484628	17 In addition to this self-associative interaction, oligomerization (dimerization) also influences the kinase activity of ROCKs by regulating its affinity for ATP. 18 Binding of active GTP-bound form of RhoA to RBD stimulates the phosphotransferase activity of ROCKs by disrupting the interaction between the catalytic and the inhibitory C-terminal region of the enzyme ( Figure 2).	bind
23435	4	6785	5	13	NULL	NULL	NULL	statement 3	Process	regulation of	leads to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_322_s_48	16484628	17 In addition to this self-associative interaction, oligomerization (dimerization) also influences the kinase activity of ROCKs by regulating its affinity for ATP. 18 Binding of active GTP-bound form of RhoA to RBD stimulates the phosphotransferase activity of ROCKs by disrupting the interaction between the catalytic and the inhibitory C-terminal region of the enzyme ( Figure 2).	bind
23436	5	6785	5	13	NULL	NULL	NULL	statement 3	Process	regulation of	leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_322_s_48	16484628	17 In addition to this self-associative interaction, oligomerization (dimerization) also influences the kinase activity of ROCKs by regulating its affinity for ATP. 18 Binding of active GTP-bound form of RhoA to RBD stimulates the phosphotransferase activity of ROCKs by disrupting the interaction between the catalytic and the inhibitory C-terminal region of the enzyme ( Figure 2).	bind
23438	6	6785	5	13	NULL	NULL	NULL	RhoA	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_322_s_48	16484628	17 In addition to this self-associative interaction, oligomerization (dimerization) also influences the kinase activity of ROCKs by regulating its affinity for ATP. 18 Binding of active GTP-bound form of RhoA to RBD stimulates the phosphotransferase activity of ROCKs by disrupting the interaction between the catalytic and the inhibitory C-terminal region of the enzyme ( Figure 2).	bind
23439	7	6785	5	13	NULL	NULL	NULL	statement 6	Process	active 	bind								RBD		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_322_s_48	16484628	17 In addition to this self-associative interaction, oligomerization (dimerization) also influences the kinase activity of ROCKs by regulating its affinity for ATP. 18 Binding of active GTP-bound form of RhoA to RBD stimulates the phosphotransferase activity of ROCKs by disrupting the interaction between the catalytic and the inhibitory C-terminal region of the enzyme ( Figure 2).	bind
23440	8	6785	5	13	NULL	NULL	NULL	statement 7	Process		stimulates					ROCKs	GP	phosphotransferase activity of 			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_322_s_48	16484628	17 In addition to this self-associative interaction, oligomerization (dimerization) also influences the kinase activity of ROCKs by regulating its affinity for ATP. 18 Binding of active GTP-bound form of RhoA to RBD stimulates the phosphotransferase activity of ROCKs by disrupting the interaction between the catalytic and the inhibitory C-terminal region of the enzyme ( Figure 2).	bind
23441	9	6785	5	13	NULL	NULL	NULL	ROCKs	GP		interacts with			catalytic C-terminal region		ROCKs	GP		inhibitory C-terminal region		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_322_s_48	16484628	17 In addition to this self-associative interaction, oligomerization (dimerization) also influences the kinase activity of ROCKs by regulating its affinity for ATP. 18 Binding of active GTP-bound form of RhoA to RBD stimulates the phosphotransferase activity of ROCKs by disrupting the interaction between the catalytic and the inhibitory C-terminal region of the enzyme ( Figure 2).	bind
23442	10	6785	5	13	NULL	NULL	NULL	statement 9	Process	disruption of	leads to					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_322_s_48	16484628	17 In addition to this self-associative interaction, oligomerization (dimerization) also influences the kinase activity of ROCKs by regulating its affinity for ATP. 18 Binding of active GTP-bound form of RhoA to RBD stimulates the phosphotransferase activity of ROCKs by disrupting the interaction between the catalytic and the inhibitory C-terminal region of the enzyme ( Figure 2).	bind
19672	1	6785	6	NULL	NULL	0	NULL	oligomerization (dimerization)	NULL		influences	NULL				ROCKs	NULL	kinase activity of			NULL		0	NULL	NULL	NULL	gw70_circulationres_98_3_322_s_48	16484628	17 In addition to this self-associative interaction, oligomerization (dimerization) also influences the kinase activity of ROCKs by regulating its affinity for ATP. 18 Binding of active GTP-bound form of RhoA to RBD stimulates the phosphotransferase activity of ROCKs by disrupting the interaction between the catalytic and the inhibitory C-terminal region of the enzyme ( Figure 2).	bind
19673	2	6785	6	NULL	NULL	0	NULL	ROCK	NULL		has affinity for	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_3_322_s_48	16484628	17 In addition to this self-associative interaction, oligomerization (dimerization) also influences the kinase activity of ROCKs by regulating its affinity for ATP. 18 Binding of active GTP-bound form of RhoA to RBD stimulates the phosphotransferase activity of ROCKs by disrupting the interaction between the catalytic and the inhibitory C-terminal region of the enzyme ( Figure 2).	bind
19674	4	6785	6	10	NULL	0	NULL	statement 3	NULL	active 	bind	NULL					NULL		RBD		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_322_s_48	16484628	17 In addition to this self-associative interaction, oligomerization (dimerization) also influences the kinase activity of ROCKs by regulating its affinity for ATP. 18 Binding of active GTP-bound form of RhoA to RBD stimulates the phosphotransferase activity of ROCKs by disrupting the interaction between the catalytic and the inhibitory C-terminal region of the enzyme ( Figure 2).	bind
19675	5	6785	6	10	NULL	0	NULL	statement 4	NULL		stimulates	NULL				ROCKs	NULL	phosphotransferase activity of 			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_322_s_48	16484628	17 In addition to this self-associative interaction, oligomerization (dimerization) also influences the kinase activity of ROCKs by regulating its affinity for ATP. 18 Binding of active GTP-bound form of RhoA to RBD stimulates the phosphotransferase activity of ROCKs by disrupting the interaction between the catalytic and the inhibitory C-terminal region of the enzyme ( Figure 2).	bind
19676	6	6785	6	10	NULL	0	NULL	ROCK	NULL		interacts with	NULL		catalytic region		ROCK	NULL	inhibitory	C-terminal region		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_322_s_48	16484628	17 In addition to this self-associative interaction, oligomerization (dimerization) also influences the kinase activity of ROCKs by regulating its affinity for ATP. 18 Binding of active GTP-bound form of RhoA to RBD stimulates the phosphotransferase activity of ROCKs by disrupting the interaction between the catalytic and the inhibitory C-terminal region of the enzyme ( Figure 2).	bind
19677	7	6785	6	10	NULL	0	NULL	statement 4	NULL		disrupts	NULL				statement 6	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_322_s_48	16484628	17 In addition to this self-associative interaction, oligomerization (dimerization) also influences the kinase activity of ROCKs by regulating its affinity for ATP. 18 Binding of active GTP-bound form of RhoA to RBD stimulates the phosphotransferase activity of ROCKs by disrupting the interaction between the catalytic and the inhibitory C-terminal region of the enzyme ( Figure 2).	bind
44695	3	6785	6	10	NULL	0	NULL	GTP	NULL		bind	NULL				RhoA	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_3_322_s_48	16484628	17 In addition to this self-associative interaction, oligomerization (dimerization) also influences the kinase activity of ROCKs by regulating its affinity for ATP. 18 Binding of active GTP-bound form of RhoA to RBD stimulates the phosphotransferase activity of ROCKs by disrupting the interaction between the catalytic and the inhibitory C-terminal region of the enzyme ( Figure 2).	bind
56562	8	6785	6	10	NULL	0	NULL	self-associative interaction			influence					ROCKs		kinase activity of			NULL		0	NULL	NULL	NULL	gw70_circulationres_98_3_322_s_48	16484628	17 In addition to this self-associative interaction, oligomerization (dimerization) also influences the kinase activity of ROCKs by regulating its affinity for ATP. 18 Binding of active GTP-bound form of RhoA to RBD stimulates the phosphotransferase activity of ROCKs by disrupting the interaction between the catalytic and the inhibitory C-terminal region of the enzyme ( Figure 2).	bind
56563	9	6785	6	10	NULL	0	NULL	statement 2		regulation of	leads to					statement 1					NULL		0	NULL	NULL	NULL	gw70_circulationres_98_3_322_s_48	16484628	17 In addition to this self-associative interaction, oligomerization (dimerization) also influences the kinase activity of ROCKs by regulating its affinity for ATP. 18 Binding of active GTP-bound form of RhoA to RBD stimulates the phosphotransferase activity of ROCKs by disrupting the interaction between the catalytic and the inhibitory C-terminal region of the enzyme ( Figure 2).	bind
56564	10	6785	6	10	NULL	0	NULL	statement 2		regulation of	leads to					statement 8					NULL		0	NULL	NULL	NULL	gw70_circulationres_98_3_322_s_48	16484628	17 In addition to this self-associative interaction, oligomerization (dimerization) also influences the kinase activity of ROCKs by regulating its affinity for ATP. 18 Binding of active GTP-bound form of RhoA to RBD stimulates the phosphotransferase activity of ROCKs by disrupting the interaction between the catalytic and the inhibitory C-terminal region of the enzyme ( Figure 2).	bind
23443	1	6786	5	13	NULL	NULL	NULL	sCD40L	GP		promote					platelets	Cell	aggregation of;;human			NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_24_2849_s_146	12070112	17 In addition, sCD40L has been shown to promote the aggregation of human or mouse platelets under conditions of high shear, an activity that results from sCD40L binding to GP IIb/IIa. 17 Thus, sCD40L appears to be a platelet agonist and necessary for thrombi stability under conditions of arterial shear.	bind
23444	2	6786	5	13	NULL	NULL	NULL	statement 1	Process		under conditions of					shear		high			NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_24_2849_s_146	12070112	17 In addition, sCD40L has been shown to promote the aggregation of human or mouse platelets under conditions of high shear, an activity that results from sCD40L binding to GP IIb/IIa. 17 Thus, sCD40L appears to be a platelet agonist and necessary for thrombi stability under conditions of arterial shear.	bind
23445	3	6786	5	13	NULL	NULL	NULL	sCD40L	GP		promote					platelets	Cell	aggregation of;;mouse			NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_24_2849_s_146	12070112	17 In addition, sCD40L has been shown to promote the aggregation of human or mouse platelets under conditions of high shear, an activity that results from sCD40L binding to GP IIb/IIa. 17 Thus, sCD40L appears to be a platelet agonist and necessary for thrombi stability under conditions of arterial shear.	bind
23446	4	6786	5	13	NULL	NULL	NULL	statement 3	Process		under conditions of					shear		high			NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_24_2849_s_146	12070112	17 In addition, sCD40L has been shown to promote the aggregation of human or mouse platelets under conditions of high shear, an activity that results from sCD40L binding to GP IIb/IIa. 17 Thus, sCD40L appears to be a platelet agonist and necessary for thrombi stability under conditions of arterial shear.	bind
23447	5	6786	5	13	NULL	NULL	NULL	sCD40L	GP		bind					GP IIb/IIa	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_24_2849_s_146	12070112	17 In addition, sCD40L has been shown to promote the aggregation of human or mouse platelets under conditions of high shear, an activity that results from sCD40L binding to GP IIb/IIa. 17 Thus, sCD40L appears to be a platelet agonist and necessary for thrombi stability under conditions of arterial shear.	bind
23448	6	6786	5	13	NULL	NULL	NULL	statement 5	Process		results in					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_24_2849_s_146	12070112	17 In addition, sCD40L has been shown to promote the aggregation of human or mouse platelets under conditions of high shear, an activity that results from sCD40L binding to GP IIb/IIa. 17 Thus, sCD40L appears to be a platelet agonist and necessary for thrombi stability under conditions of arterial shear.	bind
23449	7	6786	5	13	NULL	NULL	NULL	statement 5	Process		results in					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_24_2849_s_146	12070112	17 In addition, sCD40L has been shown to promote the aggregation of human or mouse platelets under conditions of high shear, an activity that results from sCD40L binding to GP IIb/IIa. 17 Thus, sCD40L appears to be a platelet agonist and necessary for thrombi stability under conditions of arterial shear.	bind
23450	8	6786	5	13	NULL	NULL	NULL	sCD40L	GP		is agonist of					platelet	Cell				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_24_2849_s_146	12070112	17 In addition, sCD40L has been shown to promote the aggregation of human or mouse platelets under conditions of high shear, an activity that results from sCD40L binding to GP IIb/IIa. 17 Thus, sCD40L appears to be a platelet agonist and necessary for thrombi stability under conditions of arterial shear.	bind
23475	9	6786	5	13	NULL	NULL	NULL	sCD40L	GP		is necessary for					thrombi stability	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_24_2849_s_146	12070112	17 In addition, sCD40L has been shown to promote the aggregation of human or mouse platelets under conditions of high shear, an activity that results from sCD40L binding to GP IIb/IIa. 17 Thus, sCD40L appears to be a platelet agonist and necessary for thrombi stability under conditions of arterial shear.	bind
23476	10	6786	5	13	NULL	NULL	NULL	statement 9	Process		under conditions of					arterial shear					NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_24_2849_s_146	12070112	17 In addition, sCD40L has been shown to promote the aggregation of human or mouse platelets under conditions of high shear, an activity that results from sCD40L binding to GP IIb/IIa. 17 Thus, sCD40L appears to be a platelet agonist and necessary for thrombi stability under conditions of arterial shear.	bind
19678	1	6786	6	NULL	NULL	0	NULL	sCD40L	NULL		bind	NULL				GP IIb/IIa	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_24_2849_s_146	12070112	17 In addition, sCD40L has been shown to promote the aggregation of human or mouse platelets under conditions of high shear, an activity that results from sCD40L binding to GP IIb/IIa. 17 Thus, sCD40L appears to be a platelet agonist and necessary for thrombi stability under conditions of arterial shear.	bind
19679	2	6786	6	10	NULL	0	NULL	sCD40L			promotes					platelets		aggregation of;;human			NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_24_2849_s_146	12070112	17 In addition, sCD40L has been shown to promote the aggregation of human or mouse platelets under conditions of high shear, an activity that results from sCD40L binding to GP IIb/IIa. 17 Thus, sCD40L appears to be a platelet agonist and necessary for thrombi stability under conditions of arterial shear.	bind
19680	3	6786	6	10	NULL	0	NULL	sCD40L			promotes					platelets		aggregation of;;mouse			NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_24_2849_s_146	12070112	17 In addition, sCD40L has been shown to promote the aggregation of human or mouse platelets under conditions of high shear, an activity that results from sCD40L binding to GP IIb/IIa. 17 Thus, sCD40L appears to be a platelet agonist and necessary for thrombi stability under conditions of arterial shear.	bind
19681	4	6786	6	NULL	NULL	0	NULL	statement 2	NULL		occurs under conditions of	NULL				shear	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_24_2849_s_146	12070112	17 In addition, sCD40L has been shown to promote the aggregation of human or mouse platelets under conditions of high shear, an activity that results from sCD40L binding to GP IIb/IIa. 17 Thus, sCD40L appears to be a platelet agonist and necessary for thrombi stability under conditions of arterial shear.	bind
19682	5	6786	6	NULL	NULL	0	NULL	statement 3	NULL		occurs under conditions of	NULL				shear	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_24_2849_s_146	12070112	17 In addition, sCD40L has been shown to promote the aggregation of human or mouse platelets under conditions of high shear, an activity that results from sCD40L binding to GP IIb/IIa. 17 Thus, sCD40L appears to be a platelet agonist and necessary for thrombi stability under conditions of arterial shear.	bind
19683	6	6786	6	10	NULL	0	NULL	sCD40L			is agonist of					platelet					NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_24_2849_s_146	12070112	17 In addition, sCD40L has been shown to promote the aggregation of human or mouse platelets under conditions of high shear, an activity that results from sCD40L binding to GP IIb/IIa. 17 Thus, sCD40L appears to be a platelet agonist and necessary for thrombi stability under conditions of arterial shear.	bind
19684	7	6786	6	NULL	NULL	0	NULL	sCD40L	NULL		is necessary for	NULL				thrombi stability	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_24_2849_s_146	12070112	17 In addition, sCD40L has been shown to promote the aggregation of human or mouse platelets under conditions of high shear, an activity that results from sCD40L binding to GP IIb/IIa. 17 Thus, sCD40L appears to be a platelet agonist and necessary for thrombi stability under conditions of arterial shear.	bind
19685	8	6786	6	NULL	NULL	0	NULL	statement 7	NULL		occurs under conditions of	NULL				arterial shear	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_24_2849_s_146	12070112	17 In addition, sCD40L has been shown to promote the aggregation of human or mouse platelets under conditions of high shear, an activity that results from sCD40L binding to GP IIb/IIa. 17 Thus, sCD40L appears to be a platelet agonist and necessary for thrombi stability under conditions of arterial shear.	bind
56565	9	6786	6	10	NULL	0	NULL	statement 1			result in					statement 2					NULL		0	NULL	NULL	NULL	gw60_circulation_105_24_2849_s_146	12070112	17 In addition, sCD40L has been shown to promote the aggregation of human or mouse platelets under conditions of high shear, an activity that results from sCD40L binding to GP IIb/IIa. 17 Thus, sCD40L appears to be a platelet agonist and necessary for thrombi stability under conditions of arterial shear.	bind
56566	10	6786	6	10	NULL	0	NULL	statement 1			result in					statement 3					NULL		0	NULL	NULL	NULL	gw60_circulation_105_24_2849_s_146	12070112	17 In addition, sCD40L has been shown to promote the aggregation of human or mouse platelets under conditions of high shear, an activity that results from sCD40L binding to GP IIb/IIa. 17 Thus, sCD40L appears to be a platelet agonist and necessary for thrombi stability under conditions of arterial shear.	bind
23477	1	6788	5	13	NULL	NULL	NULL	SMC	Cell	degenerate	limits				CArG box 	SRF	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_7_868_s_82	16614312	17 Our laboratory has provided evidence that this degenerate SMC CArG box serves to limit SRF binding, thereby restricting expression of SMC markers to cells that express high levels of SRF and/or cells like SMCs that have evolved mechanisms to enhance SRF binding to degenerate CArGs, ie, a SMC-selective transcriptional SRF cofactor.	bind
23478	2	6788	5	13	NULL	NULL	NULL	statement 1	Process		restricts					SMC markers	GP	expression of			NULL	cells expressing high levels of SRF	NULL	NULL	NULL	NULL	gw70_circulationres_98_7_868_s_82	16614312	17 Our laboratory has provided evidence that this degenerate SMC CArG box serves to limit SRF binding, thereby restricting expression of SMC markers to cells that express high levels of SRF and/or cells like SMCs that have evolved mechanisms to enhance SRF binding to degenerate CArGs, ie, a SMC-selective transcriptional SRF cofactor.	bind
28366	3	6788	5	13	NULL	NULL	NULL	statement 1	Process		restricts					SMC markers	GP	expression of			NULL	SMCs	NULL	NULL	NULL	NULL	gw70_circulationres_98_7_868_s_82	16614312	17 Our laboratory has provided evidence that this degenerate SMC CArG box serves to limit SRF binding, thereby restricting expression of SMC markers to cells that express high levels of SRF and/or cells like SMCs that have evolved mechanisms to enhance SRF binding to degenerate CArGs, ie, a SMC-selective transcriptional SRF cofactor.	bind
28367	4	6788	5	13	NULL	NULL	NULL	SRF	GP	binding of	degenerates									CArGs	NULL	SMCs	NULL	NULL	NULL	NULL	gw70_circulationres_98_7_868_s_82	16614312	17 Our laboratory has provided evidence that this degenerate SMC CArG box serves to limit SRF binding, thereby restricting expression of SMC markers to cells that express high levels of SRF and/or cells like SMCs that have evolved mechanisms to enhance SRF binding to degenerate CArGs, ie, a SMC-selective transcriptional SRF cofactor.	bind
28371	5	6788	5	13	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_7_868_s_82	16614312	17 Our laboratory has provided evidence that this degenerate SMC CArG box serves to limit SRF binding, thereby restricting expression of SMC markers to cells that express high levels of SRF and/or cells like SMCs that have evolved mechanisms to enhance SRF binding to degenerate CArGs, ie, a SMC-selective transcriptional SRF cofactor.	bind
19831	1	6788	6	10	NULL	0	NULL			degenerate	limits				CArG box	SRF		binding of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_7_868_s_82	16614312	17 Our laboratory has provided evidence that this degenerate SMC CArG box serves to limit SRF binding, thereby restricting expression of SMC markers to cells that express high levels of SRF and/or cells like SMCs that have evolved mechanisms to enhance SRF binding to degenerate CArGs, ie, a SMC-selective transcriptional SRF cofactor.	bind
20116	2	6788	6	10	NULL	0	NULL	statement 1			restricts					SMC markers		expression of			NULL	cells expressing high levels of SRF	NULL	NULL	NULL	NULL	gw70_circulationres_98_7_868_s_82	16614312	17 Our laboratory has provided evidence that this degenerate SMC CArG box serves to limit SRF binding, thereby restricting expression of SMC markers to cells that express high levels of SRF and/or cells like SMCs that have evolved mechanisms to enhance SRF binding to degenerate CArGs, ie, a SMC-selective transcriptional SRF cofactor.	bind
44696	3	6788	6	10	NULL	0	NULL	statement 1			restricts					SMC markers		expression of			NULL	SMCs	NULL	NULL	NULL	NULL	gw70_circulationres_98_7_868_s_82	16614312	17 Our laboratory has provided evidence that this degenerate SMC CArG box serves to limit SRF binding, thereby restricting expression of SMC markers to cells that express high levels of SRF and/or cells like SMCs that have evolved mechanisms to enhance SRF binding to degenerate CArGs, ie, a SMC-selective transcriptional SRF cofactor.	bind
57785	5	6788	6	10	NULL	0	NULL	statement 2			is an alternative to					statement 3					NULL		0	NULL	NULL	NULL	gw70_circulationres_98_7_868_s_82	16614312	17 Our laboratory has provided evidence that this degenerate SMC CArG box serves to limit SRF binding, thereby restricting expression of SMC markers to cells that express high levels of SRF and/or cells like SMCs that have evolved mechanisms to enhance SRF binding to degenerate CArGs, ie, a SMC-selective transcriptional SRF cofactor.	bind
57786	4	6788	6	10	NULL	0	NULL	SRF		binding of	degenerates									CArGs	NULL	SMCs	NULL	NULL	NULL	NULL	gw70_circulationres_98_7_868_s_82	16614312	17 Our laboratory has provided evidence that this degenerate SMC CArG box serves to limit SRF binding, thereby restricting expression of SMC markers to cells that express high levels of SRF and/or cells like SMCs that have evolved mechanisms to enhance SRF binding to degenerate CArGs, ie, a SMC-selective transcriptional SRF cofactor.	bind
23479	1	6789	5	13	NULL	NULL	NULL	ST2	GP		does not bind					interleukin-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_5_721_s_101	12578875	17 Subsequently, a membrane-anchored receptor form of ST2 was identified, 18 consisting of an extracellular domain identical to ST2, a transmembrane domain, and an intracellular domain, all with homology to the interleukin-1 receptor, although ST2 does not bind interleukin-1.	bind
23480	2	6789	5	13	NULL	NULL	NULL	ST2 receptor	GP	membrane-anchored 	homologous to					interleukin-1 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_5_721_s_101	12578875	17 Subsequently, a membrane-anchored receptor form of ST2 was identified, 18 consisting of an extracellular domain identical to ST2, a transmembrane domain, and an intracellular domain, all with homology to the interleukin-1 receptor, although ST2 does not bind interleukin-1.	bind
56569	3	6789	5	13	NULL	NULL	NULL	ST2 receptor	GP	membrane-anchored	consist of								 extracellular domain		NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_5_721_s_101	12578875	17 Subsequently, a membrane-anchored receptor form of ST2 was identified, 18 consisting of an extracellular domain identical to ST2, a transmembrane domain, and an intracellular domain, all with homology to the interleukin-1 receptor, although ST2 does not bind interleukin-1.	bind
56570	4	6789	5	13	NULL	NULL	NULL	ST2 receptor	GP	membrane-anchored	consist of								transmembrane domain		NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_5_721_s_101	12578875	17 Subsequently, a membrane-anchored receptor form of ST2 was identified, 18 consisting of an extracellular domain identical to ST2, a transmembrane domain, and an intracellular domain, all with homology to the interleukin-1 receptor, although ST2 does not bind interleukin-1.	bind
56572	5	6789	5	13	NULL	NULL	NULL	ST2 receptor	GP	membrane-anchored	consist of								intracellular domain		NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_5_721_s_101	12578875	17 Subsequently, a membrane-anchored receptor form of ST2 was identified, 18 consisting of an extracellular domain identical to ST2, a transmembrane domain, and an intracellular domain, all with homology to the interleukin-1 receptor, although ST2 does not bind interleukin-1.	bind
19832	1	6789	6	NULL	NULL	0	NULL	ST2	NULL		does not bind	NULL				interleukin-1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_107_5_721_s_101	12578875	17 Subsequently, a membrane-anchored receptor form of ST2 was identified, 18 consisting of an extracellular domain identical to ST2, a transmembrane domain, and an intracellular domain, all with homology to the interleukin-1 receptor, although ST2 does not bind interleukin-1.	bind
19833	2	6789	6	NULL	NULL	0	NULL	ST2 receptor	NULL	membrane-anchored	consists of	NULL					NULL		extracellular domain		NULL		0	NULL	NULL	NULL	gw60_circulation_107_5_721_s_101	12578875	17 Subsequently, a membrane-anchored receptor form of ST2 was identified, 18 consisting of an extracellular domain identical to ST2, a transmembrane domain, and an intracellular domain, all with homology to the interleukin-1 receptor, although ST2 does not bind interleukin-1.	bind
19834	3	6789	6	NULL	NULL	0	NULL	ST2 receptor	NULL	membrane-anchored	consists of	NULL					NULL		transmembrane domain		NULL		0	NULL	NULL	NULL	gw60_circulation_107_5_721_s_101	12578875	17 Subsequently, a membrane-anchored receptor form of ST2 was identified, 18 consisting of an extracellular domain identical to ST2, a transmembrane domain, and an intracellular domain, all with homology to the interleukin-1 receptor, although ST2 does not bind interleukin-1.	bind
19835	4	6789	6	NULL	NULL	0	NULL	ST2 receptor	NULL	membrane-anchored	consists of	NULL					NULL		intracellular domain		NULL		0	NULL	NULL	NULL	gw60_circulation_107_5_721_s_101	12578875	17 Subsequently, a membrane-anchored receptor form of ST2 was identified, 18 consisting of an extracellular domain identical to ST2, a transmembrane domain, and an intracellular domain, all with homology to the interleukin-1 receptor, although ST2 does not bind interleukin-1.	bind
56568	5	6789	6	10	NULL	0	NULL	ST2 receptor		membrane-anchored	is homologous to					 interleukin-1 receptor					NULL		0	NULL	NULL	NULL	gw60_circulation_107_5_721_s_101	12578875	17 Subsequently, a membrane-anchored receptor form of ST2 was identified, 18 consisting of an extracellular domain identical to ST2, a transmembrane domain, and an intracellular domain, all with homology to the interleukin-1 receptor, although ST2 does not bind interleukin-1.	bind
23481	1	6790	5	13	NULL	NULL	NULL	fibrinogen	GP		acts as								serotonin binding sites		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_861_s_192	15653564	17 Subsequently, it was postulated that fibrinogen and thrombospondin act as serotonin binding sites to anchor serotonin derivatized - platelet FV on the surface of platelets stimulated by thrombin plus convulxin.	bind
23482	2	6790	5	13	NULL	NULL	NULL	thrombospondin	GP		acts as								serotonin binding sites		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_861_s_192	15653564	17 Subsequently, it was postulated that fibrinogen and thrombospondin act as serotonin binding sites to anchor serotonin derivatized - platelet FV on the surface of platelets stimulated by thrombin plus convulxin.	bind
23483	3	6790	5	13	NULL	NULL	NULL	statement 1	GP		anchor					platelet FV	GP	serotonin derivatized			NULL	on the surface of platelets stimulated by thrombin plus convulxin	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_861_s_192	15653564	17 Subsequently, it was postulated that fibrinogen and thrombospondin act as serotonin binding sites to anchor serotonin derivatized - platelet FV on the surface of platelets stimulated by thrombin plus convulxin.	bind
23484	4	6790	5	13	NULL	NULL	NULL	statement 2	GP		anchor					platelet FV	GP	serotonin derivatized			NULL	on the surface of platelets stimulated by thrombin plus convulxin	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_861_s_192	15653564	17 Subsequently, it was postulated that fibrinogen and thrombospondin act as serotonin binding sites to anchor serotonin derivatized - platelet FV on the surface of platelets stimulated by thrombin plus convulxin.	bind
19836	1	6790	6	NULL	NULL	0	NULL	fibrinogen	NULL		acts as	NULL					NULL		serotonin binding sites		NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_861_s_192	15653564	17 Subsequently, it was postulated that fibrinogen and thrombospondin act as serotonin binding sites to anchor serotonin derivatized - platelet FV on the surface of platelets stimulated by thrombin plus convulxin.	bind
19837	2	6790	6	NULL	NULL	0	NULL	thrombospondin	NULL		acts as	NULL					NULL		serotonin binding sites		NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_861_s_192	15653564	17 Subsequently, it was postulated that fibrinogen and thrombospondin act as serotonin binding sites to anchor serotonin derivatized - platelet FV on the surface of platelets stimulated by thrombin plus convulxin.	bind
19838	3	6790	6	NULL	NULL	0	NULL	platelet FV	NULL	serotonin derivatized	anchored on	NULL				surface of platelets	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_861_s_192	15653564	17 Subsequently, it was postulated that fibrinogen and thrombospondin act as serotonin binding sites to anchor serotonin derivatized - platelet FV on the surface of platelets stimulated by thrombin plus convulxin.	bind
19839	4	6790	6	NULL	NULL	0	NULL	statement 1	NULL		anchor	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_861_s_192	15653564	17 Subsequently, it was postulated that fibrinogen and thrombospondin act as serotonin binding sites to anchor serotonin derivatized - platelet FV on the surface of platelets stimulated by thrombin plus convulxin.	bind
19840	5	6790	6	NULL	NULL	0	NULL	statement 2	NULL		anchor	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_861_s_192	15653564	17 Subsequently, it was postulated that fibrinogen and thrombospondin act as serotonin binding sites to anchor serotonin derivatized - platelet FV on the surface of platelets stimulated by thrombin plus convulxin.	bind
19841	6	6790	6	NULL	NULL	0	NULL	statement 3	NULL		stimulated by	NULL				thrombin plus convulxin	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_861_s_192	15653564	17 Subsequently, it was postulated that fibrinogen and thrombospondin act as serotonin binding sites to anchor serotonin derivatized - platelet FV on the surface of platelets stimulated by thrombin plus convulxin.	bind
23487	1	6791	5	13	NULL	NULL	NULL	SRF	GP		bind									CArG boxes	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_7_868_s_75	16614312	17 The general paradigm is that expression of CArG-dependent SMC differentiation genes requires SRF binding to CArG boxes to drive transcription.	bind
23488	3	6791	5	13	NULL	NULL	NULL	statement 2	Process		requires					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_7_868_s_75	16614312	17 The general paradigm is that expression of CArG-dependent SMC differentiation genes requires SRF binding to CArG boxes to drive transcription.	bind
23489	4	6791	5	13	NULL	NULL	NULL	statement 3	Process		drives					transcription	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_7_868_s_75	16614312	17 The general paradigm is that expression of CArG-dependent SMC differentiation genes requires SRF binding to CArG boxes to drive transcription.	bind
44697	2	6791	5	13	NULL	NULL	NULL	SMC differentiation genes	GP		depends on					CArG	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_7_868_s_75	16614312	17 The general paradigm is that expression of CArG-dependent SMC differentiation genes requires SRF binding to CArG boxes to drive transcription.	bind
19686	1	6791	6	NULL	NULL	0	NULL	SRF	NULL		bind	NULL					NULL			CArG box	NULL		0	NULL	NULL	NULL	gw70_circulationres_98_7_868_s_75	16614312	17 The general paradigm is that expression of CArG-dependent SMC differentiation genes requires SRF binding to CArG boxes to drive transcription.	bind
19687	3	6791	6	10	NULL	0	NULL	statement 2	NULL		requires	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_7_868_s_75	16614312	17 The general paradigm is that expression of CArG-dependent SMC differentiation genes requires SRF binding to CArG boxes to drive transcription.	bind
44698	2	6791	6	10	NULL	0	NULL	SMC differentiation genes	NULL		depends on	NULL				CArG	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_7_868_s_75	16614312	17 The general paradigm is that expression of CArG-dependent SMC differentiation genes requires SRF binding to CArG boxes to drive transcription.	bind
56573	4	6791	6	10	NULL	0	NULL	statement 3			drives					transcription					NULL		0	NULL	NULL	NULL	gw70_circulationres_98_7_868_s_75	16614312	17 The general paradigm is that expression of CArG-dependent SMC differentiation genes requires SRF binding to CArG boxes to drive transcription.	bind
45616	1	6792	5	13	NULL	NULL	NULL	RhoA	GP		interacts with					nuclear trafficking machinery	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_108_7_876_s_189	12874183	17 The interaction between RhoA and this nuclear trafficking machinery or ERK binding/scaffolding proteins to functionally compartmentalize ERK within the cell is not known.	bind
45617	2	6792	5	13	NULL	NULL	NULL	RhoA	GP		interacts with					ERK binding/scaffolding proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_108_7_876_s_189	12874183	17 The interaction between RhoA and this nuclear trafficking machinery or ERK binding/scaffolding proteins to functionally compartmentalize ERK within the cell is not known.	bind
19843	2	6792	6	NULL	NULL	0	NULL	RhoA	NULL		interacts with	NULL				ERK binding/scaffolding proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_108_7_876_s_189	12874183	17 The interaction between RhoA and this nuclear trafficking machinery or ERK binding/scaffolding proteins to functionally compartmentalize ERK within the cell is not known.	bind
44833	1	6792	6	10	NULL	0	NULL	RhoA	NULL		interact with	NULL				\tnuclear trafficking machinery	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_108_7_876_s_189	12874183	17 The interaction between RhoA and this nuclear trafficking machinery or ERK binding/scaffolding proteins to functionally compartmentalize ERK within the cell is not known.	bind
23490	1	6793	5	13	NULL	NULL	NULL	apoA-I	GP		bind		directly			ABCA1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_32	12738681	17 These findings led us to suggest that apoA-I directly binds ABCA1 to form a complex that is required for ABCA1-facilitated cellular cholesterol and phospholipid efflux.	bind
23491	2	6793	5	13	NULL	NULL	NULL	 ABCA1	GP		facilitate					cellular cholesterol efflux	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_32	12738681	17 These findings led us to suggest that apoA-I directly binds ABCA1 to form a complex that is required for ABCA1-facilitated cellular cholesterol and phospholipid efflux.	bind
23492	4	6793	5	13	NULL	NULL	NULL	statement 1	Process		is required for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_32	12738681	17 These findings led us to suggest that apoA-I directly binds ABCA1 to form a complex that is required for ABCA1-facilitated cellular cholesterol and phospholipid efflux.	bind
44699	3	6793	5	13	NULL	NULL	NULL	ABCA1	GP		facilitate					phospholipid efflux	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_32	12738681	17 These findings led us to suggest that apoA-I directly binds ABCA1 to form a complex that is required for ABCA1-facilitated cellular cholesterol and phospholipid efflux.	bind
44700	5	6793	5	13	NULL	NULL	NULL	statement 1	Process		is required for					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_32	12738681	17 These findings led us to suggest that apoA-I directly binds ABCA1 to form a complex that is required for ABCA1-facilitated cellular cholesterol and phospholipid efflux.	bind
19688	1	6793	6	NULL	NULL	0	NULL	apoA-I	NULL		bind	NULL	directly			ABCA1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_32	12738681	17 These findings led us to suggest that apoA-I directly binds ABCA1 to form a complex that is required for ABCA1-facilitated cellular cholesterol and phospholipid efflux.	bind
19689	2	6793	6	NULL	NULL	0	NULL	ABCA-1	NULL		facilitate	NULL				cellular cholesterol efflux	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_32	12738681	17 These findings led us to suggest that apoA-I directly binds ABCA1 to form a complex that is required for ABCA1-facilitated cellular cholesterol and phospholipid efflux.	bind
19690	3	6793	6	NULL	NULL	0	NULL	ABCA-1	NULL		facilitate	NULL				phospholipid efflux	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_32	12738681	17 These findings led us to suggest that apoA-I directly binds ABCA1 to form a complex that is required for ABCA1-facilitated cellular cholesterol and phospholipid efflux.	bind
19691	4	6793	6	NULL	NULL	0	NULL	statement 1	NULL		is required for	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_32	12738681	17 These findings led us to suggest that apoA-I directly binds ABCA1 to form a complex that is required for ABCA1-facilitated cellular cholesterol and phospholipid efflux.	bind
19692	5	6793	6	NULL	NULL	0	NULL	statement 1	NULL		is required for	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_32	12738681	17 These findings led us to suggest that apoA-I directly binds ABCA1 to form a complex that is required for ABCA1-facilitated cellular cholesterol and phospholipid efflux.	bind
28374	1	6794	5	13	NULL	NULL	NULL	oxLDL	GP		bind					FcgammaRII-B2	GP	murine			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3248_s_188	9409319	17 Thus, amino acid sequence differences in the IgG ligand-binding sites between both receptors could explain the discrepancy in oxLDL binding between murine FcgammaRII-B2 and human FcgammaRIIA.	bind
28375	2	6794	5	13	NULL	NULL	NULL	oxLDL	GP		bind					FcgammaRIIA	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3248_s_188	9409319	17 Thus, amino acid sequence differences in the IgG ligand-binding sites between both receptors could explain the discrepancy in oxLDL binding between murine FcgammaRII-B2 and human FcgammaRIIA.	bind
28376	3	6794	5	13	NULL	NULL	NULL	statement 1	Process		is discrepant to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3248_s_188	9409319	17 Thus, amino acid sequence differences in the IgG ligand-binding sites between both receptors could explain the discrepancy in oxLDL binding between murine FcgammaRII-B2 and human FcgammaRIIA.	bind
28377	4	6794	5	13	NULL	NULL	NULL	FcgammaRII-B2	GP	amino acid sequence of murine	differs from			IgG ligand-binding sites		FcgammaRIIA	GP	amino acid sequence of human	IgG ligand-binding sites		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3248_s_188	9409319	17 Thus, amino acid sequence differences in the IgG ligand-binding sites between both receptors could explain the discrepancy in oxLDL binding between murine FcgammaRII-B2 and human FcgammaRIIA.	bind
28378	5	6794	5	13	NULL	NULL	NULL	statement 4	Process		explains					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3248_s_188	9409319	17 Thus, amino acid sequence differences in the IgG ligand-binding sites between both receptors could explain the discrepancy in oxLDL binding between murine FcgammaRII-B2 and human FcgammaRIIA.	bind
19693	1	6794	6	NULL	NULL	0	NULL	oxLDL	NULL		bind	NULL				FcgammaRII-B2	NULL	murine			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3248_s_188	9409319	17 Thus, amino acid sequence differences in the IgG ligand-binding sites between both receptors could explain the discrepancy in oxLDL binding between murine FcgammaRII-B2 and human FcgammaRIIA.	bind
19694	2	6794	6	NULL	NULL	0	NULL	oxLDL	NULL		bind	NULL				FcgammaRIIA	NULL	human			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3248_s_188	9409319	17 Thus, amino acid sequence differences in the IgG ligand-binding sites between both receptors could explain the discrepancy in oxLDL binding between murine FcgammaRII-B2 and human FcgammaRIIA.	bind
56574	3	6794	6	10	NULL	0	NULL	statement 1			discrepant to					statement 2					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3248_s_188	9409319	17 Thus, amino acid sequence differences in the IgG ligand-binding sites between both receptors could explain the discrepancy in oxLDL binding between murine FcgammaRII-B2 and human FcgammaRIIA.	bind
56575	4	6794	6	10	NULL	0	NULL	FcgammaRII-B2		amino acid sequence of murine	differs from			 IgG ligand-binding sites		FcgammaRIIA		amino acid sequence of human	IgG ligand-binding sites		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3248_s_188	9409319	17 Thus, amino acid sequence differences in the IgG ligand-binding sites between both receptors could explain the discrepancy in oxLDL binding between murine FcgammaRII-B2 and human FcgammaRIIA.	bind
56576	5	6794	6	10	NULL	0	NULL	statement 4			explains					statement 3					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3248_s_188	9409319	17 Thus, amino acid sequence differences in the IgG ligand-binding sites between both receptors could explain the discrepancy in oxLDL binding between murine FcgammaRII-B2 and human FcgammaRIIA.	bind
23495	1	6795	5	13	NULL	NULL	NULL	Tie2	GP		bind					Dok-R	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_6_630_s_27	12609966	17 Tie2 binding with Dok-R mediates the effects of the receptor on endothelial migration.	bind
23496	2	6795	5	13	NULL	NULL	NULL	statement 1	Process		mediates					endothelial migration	Process	effects on			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_6_630_s_27	12609966	17 Tie2 binding with Dok-R mediates the effects of the receptor on endothelial migration.	bind
19695	1	6795	6	NULL	NULL	0	NULL	Tie2	NULL		bind	NULL				Dok-R	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_92_6_630_s_27	12609966	17 Tie2 binding with Dok-R mediates the effects of the receptor on endothelial migration.	bind
19696	2	6795	6	NULL	NULL	0	NULL	statement 1	NULL		mediates	NULL				endothelial migration	NULL	effects on			NULL		0	NULL	NULL	NULL	gw60_circulationres_92_6_630_s_27	12609966	17 Tie2 binding with Dok-R mediates the effects of the receptor on endothelial migration.	bind
23497	1	6796	5	13	NULL	NULL	NULL	FAK	GP		mediate					ERK	GP	downstream activation of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_37_34391_s_257	12110680	17,  18,  31,  43), the beta4-mCLCA1-triggered, FAK-mediated downstream activation of ERK is closely associated with increased rates of proliferation and BrdUrd incorporation of B16-F10 cells bound to mCLCA1-coated dishes as well as the clonal growth of tumor cells bound to BAEC monolayers that constitutively express bCLCA2 ( 5).	bind
23498	2	6796	5	13	NULL	NULL	NULL	beta4-mCLCA1	GP		triggers					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_37_34391_s_257	12110680	17,  18,  31,  43), the beta4-mCLCA1-triggered, FAK-mediated downstream activation of ERK is closely associated with increased rates of proliferation and BrdUrd incorporation of B16-F10 cells bound to mCLCA1-coated dishes as well as the clonal growth of tumor cells bound to BAEC monolayers that constitutively express bCLCA2 ( 5).	bind
23499	3	6796	5	13	NULL	NULL	NULL	statement 2	Process		is associated with		closely			B16-F10 cells 	Cell	increased rates of proliferation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_37_34391_s_257	12110680	17,  18,  31,  43), the beta4-mCLCA1-triggered, FAK-mediated downstream activation of ERK is closely associated with increased rates of proliferation and BrdUrd incorporation of B16-F10 cells bound to mCLCA1-coated dishes as well as the clonal growth of tumor cells bound to BAEC monolayers that constitutively express bCLCA2 ( 5).	bind
23500	4	6796	5	13	NULL	NULL	NULL	statement 2	Process		is associated with		closely			B16-F10 cells	Cell	BrdUrd incorporation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_37_34391_s_257	12110680	17,  18,  31,  43), the beta4-mCLCA1-triggered, FAK-mediated downstream activation of ERK is closely associated with increased rates of proliferation and BrdUrd incorporation of B16-F10 cells bound to mCLCA1-coated dishes as well as the clonal growth of tumor cells bound to BAEC monolayers that constitutively express bCLCA2 ( 5).	bind
23501	5	6796	5	13	NULL	NULL	NULL	BAEC monolayers	Cell		express		constitutively			bCLCA2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_37_34391_s_257	12110680	17,  18,  31,  43), the beta4-mCLCA1-triggered, FAK-mediated downstream activation of ERK is closely associated with increased rates of proliferation and BrdUrd incorporation of B16-F10 cells bound to mCLCA1-coated dishes as well as the clonal growth of tumor cells bound to BAEC monolayers that constitutively express bCLCA2 ( 5).	bind
23502	6	6796	5	13	NULL	NULL	NULL	tumor cells	Cell		bind					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_37_34391_s_257	12110680	17,  18,  31,  43), the beta4-mCLCA1-triggered, FAK-mediated downstream activation of ERK is closely associated with increased rates of proliferation and BrdUrd incorporation of B16-F10 cells bound to mCLCA1-coated dishes as well as the clonal growth of tumor cells bound to BAEC monolayers that constitutively express bCLCA2 ( 5).	bind
23503	7	6796	5	13	NULL	NULL	NULL	statement 2	Process		is associated with		closely			statement 6	Process	clonal growth of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_37_34391_s_257	12110680	17,  18,  31,  43), the beta4-mCLCA1-triggered, FAK-mediated downstream activation of ERK is closely associated with increased rates of proliferation and BrdUrd incorporation of B16-F10 cells bound to mCLCA1-coated dishes as well as the clonal growth of tumor cells bound to BAEC monolayers that constitutively express bCLCA2 ( 5).	bind
19844	1	6796	6	NULL	NULL	0	NULL	BAEC monolayers	NULL		express	NULL	constitutively			bCLCA2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_37_34391_s_257	12110680	17,  18,  31,  43), the beta4-mCLCA1-triggered, FAK-mediated downstream activation of ERK is closely associated with increased rates of proliferation and BrdUrd incorporation of B16-F10 cells bound to mCLCA1-coated dishes as well as the clonal growth of tumor cells bound to BAEC monolayers that constitutively express bCLCA2 ( 5).	bind
19845	2	6796	6	NULL	NULL	0	NULL	tumor cells	NULL		bind	NULL				BAEC monolayers	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_37_34391_s_257	12110680	17,  18,  31,  43), the beta4-mCLCA1-triggered, FAK-mediated downstream activation of ERK is closely associated with increased rates of proliferation and BrdUrd incorporation of B16-F10 cells bound to mCLCA1-coated dishes as well as the clonal growth of tumor cells bound to BAEC monolayers that constitutively express bCLCA2 ( 5).	bind
19846	3	6796	6	NULL	NULL	0	NULL	FAK	NULL		mediates	NULL				ERK	NULL	downstream activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_37_34391_s_257	12110680	17,  18,  31,  43), the beta4-mCLCA1-triggered, FAK-mediated downstream activation of ERK is closely associated with increased rates of proliferation and BrdUrd incorporation of B16-F10 cells bound to mCLCA1-coated dishes as well as the clonal growth of tumor cells bound to BAEC monolayers that constitutively express bCLCA2 ( 5).	bind
19847	6	6796	6	10	NULL	0	NULL	statement 4			is associated with					B16-F10 cells 		increased rate of proliferation			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_37_34391_s_257	12110680	17,  18,  31,  43), the beta4-mCLCA1-triggered, FAK-mediated downstream activation of ERK is closely associated with increased rates of proliferation and BrdUrd incorporation of B16-F10 cells bound to mCLCA1-coated dishes as well as the clonal growth of tumor cells bound to BAEC monolayers that constitutively express bCLCA2 ( 5).	bind
19848	5	6796	6	10	NULL	0	NULL	statement 4			is associated with					statement 2		clonal growth of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_37_34391_s_257	12110680	17,  18,  31,  43), the beta4-mCLCA1-triggered, FAK-mediated downstream activation of ERK is closely associated with increased rates of proliferation and BrdUrd incorporation of B16-F10 cells bound to mCLCA1-coated dishes as well as the clonal growth of tumor cells bound to BAEC monolayers that constitutively express bCLCA2 ( 5).	bind
20300	4	6796	6	10	NULL	0	NULL	beta4-mCLCA1			triggers					statement 3					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_37_34391_s_257	12110680	17,  18,  31,  43), the beta4-mCLCA1-triggered, FAK-mediated downstream activation of ERK is closely associated with increased rates of proliferation and BrdUrd incorporation of B16-F10 cells bound to mCLCA1-coated dishes as well as the clonal growth of tumor cells bound to BAEC monolayers that constitutively express bCLCA2 ( 5).	bind
56577	7	6796	6	10	NULL	0	NULL	statement 4			associated with		closely			B16-F10 cells 		BrdUrd incorporation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_37_34391_s_257	12110680	17,  18,  31,  43), the beta4-mCLCA1-triggered, FAK-mediated downstream activation of ERK is closely associated with increased rates of proliferation and BrdUrd incorporation of B16-F10 cells bound to mCLCA1-coated dishes as well as the clonal growth of tumor cells bound to BAEC monolayers that constitutively express bCLCA2 ( 5).	bind
23504	1	6797	5	13	NULL	NULL	NULL	VEGF	GP		bind					VEGFR-2/Flk1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1124_s_217	15044320	17,18  In physiological angiogenesis, the net levels of VEGF binding to VEGFR-2/Flk1 are regulated by competing levels of VEGFR-1/Flt1, thereby preventing aberrant activation of VEGFR-2/Flk1.	bind
23505	2	6797	5	13	NULL	NULL	NULL	VEGF	GP		bind					VEGFR-1/Flt1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1124_s_217	15044320	17,18  In physiological angiogenesis, the net levels of VEGF binding to VEGFR-2/Flk1 are regulated by competing levels of VEGFR-1/Flt1, thereby preventing aberrant activation of VEGFR-2/Flk1.	bind
23506	3	6797	5	13	NULL	NULL	NULL	statement 2	Process		competes with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1124_s_217	15044320	17,18  In physiological angiogenesis, the net levels of VEGF binding to VEGFR-2/Flk1 are regulated by competing levels of VEGFR-1/Flt1, thereby preventing aberrant activation of VEGFR-2/Flk1.	bind
23507	4	6797	5	13	NULL	NULL	NULL	statement 1	Process	levels of	is regulated by					statement 3	Process				NULL	in physiological angiogenesis	NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1124_s_217	15044320	17,18  In physiological angiogenesis, the net levels of VEGF binding to VEGFR-2/Flk1 are regulated by competing levels of VEGFR-1/Flt1, thereby preventing aberrant activation of VEGFR-2/Flk1.	bind
23508	5	6797	5	13	NULL	NULL	NULL	statement 4	Process		prevents					VEGFR-2/Flk1	GP	aberrant activation of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1124_s_217	15044320	17,18  In physiological angiogenesis, the net levels of VEGF binding to VEGFR-2/Flk1 are regulated by competing levels of VEGFR-1/Flt1, thereby preventing aberrant activation of VEGFR-2/Flk1.	bind
19849	1	6797	6	NULL	NULL	0	NULL	VEGF	NULL		bind	NULL				VEGFR-2/Flk1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_8_1124_s_217	15044320	17,18  In physiological angiogenesis, the net levels of VEGF binding to VEGFR-2/Flk1 are regulated by competing levels of VEGFR-1/Flt1, thereby preventing aberrant activation of VEGFR-2/Flk1.	bind
19850	2	6797	6	10	NULL	0	NULL	VEGF			bind					VEGFR-1/Flt1					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1124_s_217	15044320	17,18  In physiological angiogenesis, the net levels of VEGF binding to VEGFR-2/Flk1 are regulated by competing levels of VEGFR-1/Flt1, thereby preventing aberrant activation of VEGFR-2/Flk1.	bind
56578	3	6797	6	10	NULL	0	NULL	statement 2			compete with					statement 3					NULL		0	NULL	NULL	NULL	gw70_circulationres_94_8_1124_s_217	15044320	17,18  In physiological angiogenesis, the net levels of VEGF binding to VEGFR-2/Flk1 are regulated by competing levels of VEGFR-1/Flt1, thereby preventing aberrant activation of VEGFR-2/Flk1.	bind
56579	4	6797	6	10	NULL	0	NULL	statement 3			regulates					statement 1		levels of			NULL	physiological angiogenesis	NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1124_s_217	15044320	17,18  In physiological angiogenesis, the net levels of VEGF binding to VEGFR-2/Flk1 are regulated by competing levels of VEGFR-1/Flt1, thereby preventing aberrant activation of VEGFR-2/Flk1.	bind
56580	5	6797	6	10	NULL	0	NULL	statement 4			prevents					VEGFR-2/Flk1		aberrant activation of			NULL		0	NULL	NULL	NULL	gw70_circulationres_94_8_1124_s_217	15044320	17,18  In physiological angiogenesis, the net levels of VEGF binding to VEGFR-2/Flk1 are regulated by competing levels of VEGFR-1/Flt1, thereby preventing aberrant activation of VEGFR-2/Flk1.	bind
23509	1	6798	5	13	NULL	NULL	NULL	MCP-1	GP	mutant	bind					CCR2 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_534_s_34	14739122	17,18  This mutant MCP-1 binds to its receptor CCR2 and blocks MCP-1 - mediated monocyte chemotaxis.	bind
23510	2	6798	5	13	NULL	NULL	NULL	MCP-1	GP		mediate					monocyte chemotaxis	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_534_s_34	14739122	17,18  This mutant MCP-1 binds to its receptor CCR2 and blocks MCP-1 - mediated monocyte chemotaxis.	bind
23511	3	6798	5	13	NULL	NULL	NULL	statement 1	Process		blocks					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_534_s_34	14739122	17,18  This mutant MCP-1 binds to its receptor CCR2 and blocks MCP-1 - mediated monocyte chemotaxis.	bind
19697	1	6798	6	NULL	NULL	0	NULL	MCP-1	NULL	mutant	bind	NULL				CCR2 receptor	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_534_s_34	14739122	17,18  This mutant MCP-1 binds to its receptor CCR2 and blocks MCP-1 - mediated monocyte chemotaxis.	bind
19698	2	6798	6	NULL	NULL	0	NULL	MCP-1	NULL		mediates	NULL				monocyte chemotaxis	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_534_s_34	14739122	17,18  This mutant MCP-1 binds to its receptor CCR2 and blocks MCP-1 - mediated monocyte chemotaxis.	bind
19699	3	6798	6	NULL	NULL	0	NULL	statement 1	NULL		blocks	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_534_s_34	14739122	17,18  This mutant MCP-1 binds to its receptor CCR2 and blocks MCP-1 - mediated monocyte chemotaxis.	bind
23512	1	6799	5	13	NULL	NULL	NULL	Stat3	GP	activation	is dependent on					Rac1	GP				NULL	 in epidermal growth factor - stimulated COS-1 cells	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1395_s_149	15860735	17,19  Stat3 activation has been shown to be Rac1 dependent in epidermal growth factor - stimulated COS-1 cells, 20 attributed to direct binding of Rac1 to Stat3 or indirect enhancement of ROS production by Rac1.	bind
23513	2	6799	5	13	NULL	NULL	NULL	Rac1	GP		bind		directly			Stat3	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1395_s_149	15860735	17,19  Stat3 activation has been shown to be Rac1 dependent in epidermal growth factor - stimulated COS-1 cells, 20 attributed to direct binding of Rac1 to Stat3 or indirect enhancement of ROS production by Rac1.	bind
23514	3	6799	5	13	NULL	NULL	NULL	statement 1	Process		is attributed to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1395_s_149	15860735	17,19  Stat3 activation has been shown to be Rac1 dependent in epidermal growth factor - stimulated COS-1 cells, 20 attributed to direct binding of Rac1 to Stat3 or indirect enhancement of ROS production by Rac1.	bind
23515	4	6799	5	13	NULL	NULL	NULL	Rac1	GP		enhances		indirectly			ROS	Chemical	production of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1395_s_149	15860735	17,19  Stat3 activation has been shown to be Rac1 dependent in epidermal growth factor - stimulated COS-1 cells, 20 attributed to direct binding of Rac1 to Stat3 or indirect enhancement of ROS production by Rac1.	bind
23516	5	6799	5	13	NULL	NULL	NULL	statement 1	Process		is attributed to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1395_s_149	15860735	17,19  Stat3 activation has been shown to be Rac1 dependent in epidermal growth factor - stimulated COS-1 cells, 20 attributed to direct binding of Rac1 to Stat3 or indirect enhancement of ROS production by Rac1.	bind
19851	1	6799	6	NULL	NULL	0	NULL	Stat3	NULL	activation of	is dependent on	NULL				Rac1	NULL				NULL	epidermal growth factor - stimulated COS-1 cells	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1395_s_149	15860735	17,19  Stat3 activation has been shown to be Rac1 dependent in epidermal growth factor - stimulated COS-1 cells, 20 attributed to direct binding of Rac1 to Stat3 or indirect enhancement of ROS production by Rac1.	bind
19852	2	6799	6	NULL	NULL	0	NULL	Rac1	NULL		bind	NULL	directly			Stat3	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1395_s_149	15860735	17,19  Stat3 activation has been shown to be Rac1 dependent in epidermal growth factor - stimulated COS-1 cells, 20 attributed to direct binding of Rac1 to Stat3 or indirect enhancement of ROS production by Rac1.	bind
19853	3	6799	6	NULL	NULL	0	NULL	Rac1	NULL		enhances	NULL	indirectly			ROS	NULL	production of 			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1395_s_149	15860735	17,19  Stat3 activation has been shown to be Rac1 dependent in epidermal growth factor - stimulated COS-1 cells, 20 attributed to direct binding of Rac1 to Stat3 or indirect enhancement of ROS production by Rac1.	bind
56581	4	6799	6	10	NULL	0	NULL	statement 1			attributed to					statement 2					NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1395_s_149	15860735	17,19  Stat3 activation has been shown to be Rac1 dependent in epidermal growth factor - stimulated COS-1 cells, 20 attributed to direct binding of Rac1 to Stat3 or indirect enhancement of ROS production by Rac1.	bind
56582	5	6799	6	10	NULL	0	NULL	statement 1			attributed to					statement 3					NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1395_s_149	15860735	17,19  Stat3 activation has been shown to be Rac1 dependent in epidermal growth factor - stimulated COS-1 cells, 20 attributed to direct binding of Rac1 to Stat3 or indirect enhancement of ROS production by Rac1.	bind
23517	1	6800	5	13	NULL	NULL	NULL	calmodulin	GP		bind					eNOS	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2238_s_30	15486309	17,20  Furthermore, Hsp90 may mediate eNOS phosphorylation through regulating calmodulin binding to eNOS and Akt. 18,19,21	bind
23518	2	6800	5	13	NULL	NULL	NULL	calmodulin	GP		bind					Akt	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2238_s_30	15486309	17,20  Furthermore, Hsp90 may mediate eNOS phosphorylation through regulating calmodulin binding to eNOS and Akt. 18,19,21	bind
23519	3	6800	5	13	NULL	NULL	NULL	Hsp90	GP		regulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2238_s_30	15486309	17,20  Furthermore, Hsp90 may mediate eNOS phosphorylation through regulating calmodulin binding to eNOS and Akt. 18,19,21	bind
23520	4	6800	5	13	NULL	NULL	NULL	Hsp90	GP		regulates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2238_s_30	15486309	17,20  Furthermore, Hsp90 may mediate eNOS phosphorylation through regulating calmodulin binding to eNOS and Akt. 18,19,21	bind
23521	5	6800	5	13	NULL	NULL	NULL	Hsp90	GP		mediate		may			eNOS	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2238_s_30	15486309	17,20  Furthermore, Hsp90 may mediate eNOS phosphorylation through regulating calmodulin binding to eNOS and Akt. 18,19,21	bind
23522	6	6800	5	13	NULL	NULL	NULL	statement 5	Process		occurs through					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2238_s_30	15486309	17,20  Furthermore, Hsp90 may mediate eNOS phosphorylation through regulating calmodulin binding to eNOS and Akt. 18,19,21	bind
23523	7	6800	5	13	NULL	NULL	NULL	statement 5	Process		occurs through					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2238_s_30	15486309	17,20  Furthermore, Hsp90 may mediate eNOS phosphorylation through regulating calmodulin binding to eNOS and Akt. 18,19,21	bind
19700	1	6800	6	NULL	NULL	0	NULL	Calmodulin	NULL		bind	NULL				eNOS	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2238_s_30	15486309	17,20  Furthermore, Hsp90 may mediate eNOS phosphorylation through regulating calmodulin binding to eNOS and Akt. 18,19,21	bind
19701	2	6800	6	NULL	NULL	0	NULL	Calmodulin	NULL		bind	NULL				Akt	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2238_s_30	15486309	17,20  Furthermore, Hsp90 may mediate eNOS phosphorylation through regulating calmodulin binding to eNOS and Akt. 18,19,21	bind
19702	3	6800	6	NULL	NULL	0	NULL	Hsp90	NULL		mediate	NULL	may			eNOS	NULL	phosphorylation of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2238_s_30	15486309	17,20  Furthermore, Hsp90 may mediate eNOS phosphorylation through regulating calmodulin binding to eNOS and Akt. 18,19,21	bind
19703	4	6800	6	NULL	NULL	0	NULL	Hsp90	NULL		regulate	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2238_s_30	15486309	17,20  Furthermore, Hsp90 may mediate eNOS phosphorylation through regulating calmodulin binding to eNOS and Akt. 18,19,21	bind
19704	5	6800	6	NULL	NULL	0	NULL	Hsp90	NULL		regulate	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2238_s_30	15486309	17,20  Furthermore, Hsp90 may mediate eNOS phosphorylation through regulating calmodulin binding to eNOS and Akt. 18,19,21	bind
19705	6	6800	6	NULL	NULL	0	NULL	statement 3	NULL		occurs through	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2238_s_30	15486309	17,20  Furthermore, Hsp90 may mediate eNOS phosphorylation through regulating calmodulin binding to eNOS and Akt. 18,19,21	bind
19706	7	6800	6	NULL	NULL	0	NULL	statement 3	NULL		occurs through	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2238_s_30	15486309	17,20  Furthermore, Hsp90 may mediate eNOS phosphorylation through regulating calmodulin binding to eNOS and Akt. 18,19,21	bind
23524	1	6801	5	13	NULL	NULL	NULL	FrzA/sFRP-1	GP		bind					Wnt	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_12_1299_s_29	15920021	17,22  We and others have shown that FrzA/sFRP-1 binds Wnt to prevent it from accessing its cell-surface receptor Frizzled, and that it blocks the canonical Wnt pathway as measured by cytosolic accumulation of beta-catenin in endothelial cells (ECs).	bind
23525	2	6801	5	13	NULL	NULL	NULL	Wnt	GP		access					Frizzled	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_12_1299_s_29	15920021	17,22  We and others have shown that FrzA/sFRP-1 binds Wnt to prevent it from accessing its cell-surface receptor Frizzled, and that it blocks the canonical Wnt pathway as measured by cytosolic accumulation of beta-catenin in endothelial cells (ECs).	bind
23526	3	6801	5	13	NULL	NULL	NULL	statement 1	Process		prevents					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_12_1299_s_29	15920021	17,22  We and others have shown that FrzA/sFRP-1 binds Wnt to prevent it from accessing its cell-surface receptor Frizzled, and that it blocks the canonical Wnt pathway as measured by cytosolic accumulation of beta-catenin in endothelial cells (ECs).	bind
23527	4	6801	5	13	NULL	NULL	NULL	statement 3	Process		blocks					 Wnt pathway	Process	canonical			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_12_1299_s_29	15920021	17,22  We and others have shown that FrzA/sFRP-1 binds Wnt to prevent it from accessing its cell-surface receptor Frizzled, and that it blocks the canonical Wnt pathway as measured by cytosolic accumulation of beta-catenin in endothelial cells (ECs).	bind
56583	5	6801	5	13	NULL	NULL	NULL	Frizzled	GP		is a type of					cell-surface receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_12_1299_s_29	15920021	17,22  We and others have shown that FrzA/sFRP-1 binds Wnt to prevent it from accessing its cell-surface receptor Frizzled, and that it blocks the canonical Wnt pathway as measured by cytosolic accumulation of beta-catenin in endothelial cells (ECs).	bind
19707	1	6801	6	NULL	NULL	0	NULL	FrzA/sFRP-1	NULL		bind	NULL				Wnt	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_12_1299_s_29	15920021	17,22  We and others have shown that FrzA/sFRP-1 binds Wnt to prevent it from accessing its cell-surface receptor Frizzled, and that it blocks the canonical Wnt pathway as measured by cytosolic accumulation of beta-catenin in endothelial cells (ECs).	bind
19708	2	6801	6	NULL	NULL	0	NULL	FrzA/sFRP-1	NULL		blocks	NULL				Wnt pathway	NULL	canonical			NULL		0	NULL	NULL	NULL	gw70_circulationres_96_12_1299_s_29	15920021	17,22  We and others have shown that FrzA/sFRP-1 binds Wnt to prevent it from accessing its cell-surface receptor Frizzled, and that it blocks the canonical Wnt pathway as measured by cytosolic accumulation of beta-catenin in endothelial cells (ECs).	bind
19709	3	6801	6	NULL	NULL	0	NULL	Wnt	NULL		access	NULL				Frizzled	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_12_1299_s_29	15920021	17,22  We and others have shown that FrzA/sFRP-1 binds Wnt to prevent it from accessing its cell-surface receptor Frizzled, and that it blocks the canonical Wnt pathway as measured by cytosolic accumulation of beta-catenin in endothelial cells (ECs).	bind
19710	4	6801	6	10	NULL	0	NULL	frizzled			is a type of					cell-surface receptor					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_12_1299_s_29	15920021	17,22  We and others have shown that FrzA/sFRP-1 binds Wnt to prevent it from accessing its cell-surface receptor Frizzled, and that it blocks the canonical Wnt pathway as measured by cytosolic accumulation of beta-catenin in endothelial cells (ECs).	bind
19711	5	6801	6	NULL	NULL	0	NULL	statement 1	NULL		prevents	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_12_1299_s_29	15920021	17,22  We and others have shown that FrzA/sFRP-1 binds Wnt to prevent it from accessing its cell-surface receptor Frizzled, and that it blocks the canonical Wnt pathway as measured by cytosolic accumulation of beta-catenin in endothelial cells (ECs).	bind
23529	1	6802	5	13	NULL	NULL	NULL	sPLA2-IIA proteins	GP		does not bind					proteoglycans	GP	mutant b3E			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1161_s_224	15802623	17,33  Our results using cell supernatant containing sPLA2-IIA proteins unable to bind proteoglycans (mutant b3E) demonstrated the involvement of proteoglycan interactions in the induction of sPLA2-IIA gene transcription.	bind
23530	2	6802	5	13	NULL	NULL	NULL	proteoglycan	GP	interactions	is involved in					sPLA2-IIA gene	GP	induction of;;transcription of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1161_s_224	15802623	17,33  Our results using cell supernatant containing sPLA2-IIA proteins unable to bind proteoglycans (mutant b3E) demonstrated the involvement of proteoglycan interactions in the induction of sPLA2-IIA gene transcription.	bind
23532	3	6802	5	13	NULL	NULL	NULL	statement 1	Process		demonstrate					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1161_s_224	15802623	17,33  Our results using cell supernatant containing sPLA2-IIA proteins unable to bind proteoglycans (mutant b3E) demonstrated the involvement of proteoglycan interactions in the induction of sPLA2-IIA gene transcription.	bind
19712	1	6802	6	10	NULL	0	NULL	sPLA2-IIA protein	NULL		does not bind	NULL				proteoglycans	NULL	mutant b3E			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1161_s_224	15802623	17,33  Our results using cell supernatant containing sPLA2-IIA proteins unable to bind proteoglycans (mutant b3E) demonstrated the involvement of proteoglycan interactions in the induction of sPLA2-IIA gene transcription.	bind
19713	2	6802	6	10	NULL	0	NULL	proteoglycan 		interactions	plays a role in					sPLA2-IIA gene		induction of;;transcription of 			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1161_s_224	15802623	17,33  Our results using cell supernatant containing sPLA2-IIA proteins unable to bind proteoglycans (mutant b3E) demonstrated the involvement of proteoglycan interactions in the induction of sPLA2-IIA gene transcription.	bind
56584	3	6802	6	10	NULL	0	NULL	statement 1			demonstrate					statement 2					NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1161_s_224	15802623	17,33  Our results using cell supernatant containing sPLA2-IIA proteins unable to bind proteoglycans (mutant b3E) demonstrated the involvement of proteoglycan interactions in the induction of sPLA2-IIA gene transcription.	bind
23531	1	6803	5	13	NULL	NULL	NULL	LRP-1B	GP		is similar to					LRP-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_6_1246_s_100	16574889	17,68 - 70    LRP-1B is the giant family member that is most similar to LRP-1; it also binds to the PDGF beta-receptor and modulates receptor-mediated signaling in SMCs. 23 These findings suggest that SMC migration might be regulated by the time-restricted expression of LRs, which determines the outcome of PDGF beta-receptor -  and uPA receptor - mediated signaling.	bind
23533	2	6803	5	13	NULL	NULL	NULL	LRP-1B	GP		bind					PDGF beta-receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_6_1246_s_100	16574889	17,68 - 70    LRP-1B is the giant family member that is most similar to LRP-1; it also binds to the PDGF beta-receptor and modulates receptor-mediated signaling in SMCs. 23 These findings suggest that SMC migration might be regulated by the time-restricted expression of LRs, which determines the outcome of PDGF beta-receptor -  and uPA receptor - mediated signaling.	bind
23534	3	6803	5	13	NULL	NULL	NULL	LRP-1B	GP		modulates					receptor-mediated signaling	Process				NULL	in SMCs	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_6_1246_s_100	16574889	17,68 - 70    LRP-1B is the giant family member that is most similar to LRP-1; it also binds to the PDGF beta-receptor and modulates receptor-mediated signaling in SMCs. 23 These findings suggest that SMC migration might be regulated by the time-restricted expression of LRs, which determines the outcome of PDGF beta-receptor -  and uPA receptor - mediated signaling.	bind
23535	5	6803	5	13	NULL	NULL	NULL	statement 4	Process		determines					PDGF beta-receptor mediated signaling	Process	outcome of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_6_1246_s_100	16574889	17,68 - 70    LRP-1B is the giant family member that is most similar to LRP-1; it also binds to the PDGF beta-receptor and modulates receptor-mediated signaling in SMCs. 23 These findings suggest that SMC migration might be regulated by the time-restricted expression of LRs, which determines the outcome of PDGF beta-receptor -  and uPA receptor - mediated signaling.	bind
23536	6	6803	5	13	NULL	NULL	NULL	statement 4	Process		determines					uPA receptor mediated signaling	Process	outcome of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_6_1246_s_100	16574889	17,68 - 70    LRP-1B is the giant family member that is most similar to LRP-1; it also binds to the PDGF beta-receptor and modulates receptor-mediated signaling in SMCs. 23 These findings suggest that SMC migration might be regulated by the time-restricted expression of LRs, which determines the outcome of PDGF beta-receptor -  and uPA receptor - mediated signaling.	bind
56586	4	6803	5	13	NULL	NULL	NULL	LRs	GP	time-restricted expression of	regulates					SMC	Cell	migration of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_6_1246_s_100	16574889	17,68 - 70    LRP-1B is the giant family member that is most similar to LRP-1; it also binds to the PDGF beta-receptor and modulates receptor-mediated signaling in SMCs. 23 These findings suggest that SMC migration might be regulated by the time-restricted expression of LRs, which determines the outcome of PDGF beta-receptor -  and uPA receptor - mediated signaling.	bind
19714	1	6803	6	NULL	NULL	0	NULL	LRP-1B	NULL		bind	NULL				PDGF beta-receptor	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_6_1246_s_100	16574889	17,68 - 70    LRP-1B is the giant family member that is most similar to LRP-1; it also binds to the PDGF beta-receptor and modulates receptor-mediated signaling in SMCs. 23 These findings suggest that SMC migration might be regulated by the time-restricted expression of LRs, which determines the outcome of PDGF beta-receptor -  and uPA receptor - mediated signaling.	bind
19715	2	6803	6	NULL	NULL	0	NULL	LRP-1B	NULL		modulates	NULL				receptor mediated signaling	NULL				NULL	SMC	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_6_1246_s_100	16574889	17,68 - 70    LRP-1B is the giant family member that is most similar to LRP-1; it also binds to the PDGF beta-receptor and modulates receptor-mediated signaling in SMCs. 23 These findings suggest that SMC migration might be regulated by the time-restricted expression of LRs, which determines the outcome of PDGF beta-receptor -  and uPA receptor - mediated signaling.	bind
19716	3	6803	6	NULL	NULL	0	NULL	LRs	NULL	time dependent expression of	regulates	NULL				SMC	NULL	migration of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_6_1246_s_100	16574889	17,68 - 70    LRP-1B is the giant family member that is most similar to LRP-1; it also binds to the PDGF beta-receptor and modulates receptor-mediated signaling in SMCs. 23 These findings suggest that SMC migration might be regulated by the time-restricted expression of LRs, which determines the outcome of PDGF beta-receptor -  and uPA receptor - mediated signaling.	bind
56585	4	6803	6	10	NULL	0	NULL	LRP-1B			is similar to					LRP-1					NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_6_1246_s_100	16574889	17,68 - 70    LRP-1B is the giant family member that is most similar to LRP-1; it also binds to the PDGF beta-receptor and modulates receptor-mediated signaling in SMCs. 23 These findings suggest that SMC migration might be regulated by the time-restricted expression of LRs, which determines the outcome of PDGF beta-receptor -  and uPA receptor - mediated signaling.	bind
56587	5	6803	6	10	NULL	0	NULL	statement 3			determines					PDGF beta-receptor mediated signaling		outcome of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_6_1246_s_100	16574889	17,68 - 70    LRP-1B is the giant family member that is most similar to LRP-1; it also binds to the PDGF beta-receptor and modulates receptor-mediated signaling in SMCs. 23 These findings suggest that SMC migration might be regulated by the time-restricted expression of LRs, which determines the outcome of PDGF beta-receptor -  and uPA receptor - mediated signaling.	bind
56588	6	6803	6	10	NULL	0	NULL	statement 3			determines					uPA receptor - mediated signaling		outcome of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_6_1246_s_100	16574889	17,68 - 70    LRP-1B is the giant family member that is most similar to LRP-1; it also binds to the PDGF beta-receptor and modulates receptor-mediated signaling in SMCs. 23 These findings suggest that SMC migration might be regulated by the time-restricted expression of LRs, which determines the outcome of PDGF beta-receptor -  and uPA receptor - mediated signaling.	bind
23537	1	6804	5	13	NULL	NULL	NULL	FasL	GP		bind					Fas protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1785_s_129	10362803	17- 19  Binding of FasL to Fas protein induces trimerization of Fas protein and FADD/MORT-1 and Daxx, the adapter proteins of Fas, bind to the trimerized Fas cytoplasmic region (death domain).	bind
23538	2	6804	5	13	NULL	NULL	NULL	statement 1	Process		induce					Fas protein	GP	trimerization of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1785_s_129	10362803	17- 19  Binding of FasL to Fas protein induces trimerization of Fas protein and FADD/MORT-1 and Daxx, the adapter proteins of Fas, bind to the trimerized Fas cytoplasmic region (death domain).	bind
23539	3	6804	5	13	NULL	NULL	NULL	FADD/MORT-1	GP		is a type of					Fas	GP	adapter protein of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1785_s_129	10362803	17- 19  Binding of FasL to Fas protein induces trimerization of Fas protein and FADD/MORT-1 and Daxx, the adapter proteins of Fas, bind to the trimerized Fas cytoplasmic region (death domain).	bind
23540	4	6804	5	13	NULL	NULL	NULL	Daxx	GP		is a type of					Fas	GP	adapter protein of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1785_s_129	10362803	17- 19  Binding of FasL to Fas protein induces trimerization of Fas protein and FADD/MORT-1 and Daxx, the adapter proteins of Fas, bind to the trimerized Fas cytoplasmic region (death domain).	bind
56589	5	6804	5	13	NULL	NULL	NULL	statement 3	GP		bind					Fas	GP	trimerized	cytoplasmic region (death domain)		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1785_s_129	10362803	17- 19  Binding of FasL to Fas protein induces trimerization of Fas protein and FADD/MORT-1 and Daxx, the adapter proteins of Fas, bind to the trimerized Fas cytoplasmic region (death domain).	bind
56590	6	6804	5	13	NULL	NULL	NULL	statement 4	GP		bind					Fas	GP	trimerized	cytoplasmic region (death domain)		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1785_s_129	10362803	17- 19  Binding of FasL to Fas protein induces trimerization of Fas protein and FADD/MORT-1 and Daxx, the adapter proteins of Fas, bind to the trimerized Fas cytoplasmic region (death domain).	bind
19717	1	6804	6	NULL	NULL	0	NULL	FasL	NULL		bind	NULL				Fas protein	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_6_1785_s_129	10362803	17- 19  Binding of FasL to Fas protein induces trimerization of Fas protein and FADD/MORT-1 and Daxx, the adapter proteins of Fas, bind to the trimerized Fas cytoplasmic region (death domain).	bind
19718	2	6804	6	NULL	NULL	0	NULL	statement 1	NULL		induces	NULL				Fas protein	NULL	trimerization of 			NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_6_1785_s_129	10362803	17- 19  Binding of FasL to Fas protein induces trimerization of Fas protein and FADD/MORT-1 and Daxx, the adapter proteins of Fas, bind to the trimerized Fas cytoplasmic region (death domain).	bind
19719	3	6804	6	10	NULL	0	NULL	FADD/MORT-1	NULL		is a type of	NULL				adapter protein of Fas	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1785_s_129	10362803	17- 19  Binding of FasL to Fas protein induces trimerization of Fas protein and FADD/MORT-1 and Daxx, the adapter proteins of Fas, bind to the trimerized Fas cytoplasmic region (death domain).	bind
19720	4	6804	6	10	NULL	0	NULL	Daxx	NULL		is a type of	NULL				adapter protein of Fas	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1785_s_129	10362803	17- 19  Binding of FasL to Fas protein induces trimerization of Fas protein and FADD/MORT-1 and Daxx, the adapter proteins of Fas, bind to the trimerized Fas cytoplasmic region (death domain).	bind
19721	5	6804	6	NULL	NULL	0	NULL	statement 3	NULL		bind	NULL				Fas	NULL	trimerized	cytoplasmic region (death domain)		NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_6_1785_s_129	10362803	17- 19  Binding of FasL to Fas protein induces trimerization of Fas protein and FADD/MORT-1 and Daxx, the adapter proteins of Fas, bind to the trimerized Fas cytoplasmic region (death domain).	bind
19722	6	6804	6	NULL	NULL	0	NULL	statement 4	NULL		bind	NULL				Fas	NULL	trimerized	cytoplasmic region (death domain)		NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_6_1785_s_129	10362803	17- 19  Binding of FasL to Fas protein induces trimerization of Fas protein and FADD/MORT-1 and Daxx, the adapter proteins of Fas, bind to the trimerized Fas cytoplasmic region (death domain).	bind
23541	1	6805	5	13	NULL	NULL	NULL	Hsp47	GP		bind		transiently			collagen type I	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_219	9686751	176  Hsp47 binds transiently to collagen types I to IV and avidly to denatured collagen substrates; thus, its role in procollagen processing and transport seems firmly established.	bind
23542	2	6805	5	13	NULL	NULL	NULL	Hsp47	GP		bind		transiently			collagen type II	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_219	9686751	176  Hsp47 binds transiently to collagen types I to IV and avidly to denatured collagen substrates; thus, its role in procollagen processing and transport seems firmly established.	bind
23543	3	6805	5	13	NULL	NULL	NULL	Hsp47	GP		bind		transiently			collagen type III	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_219	9686751	176  Hsp47 binds transiently to collagen types I to IV and avidly to denatured collagen substrates; thus, its role in procollagen processing and transport seems firmly established.	bind
23544	4	6805	5	13	NULL	NULL	NULL	Hsp47	GP		bind		transiently			collagen type IV	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_219	9686751	176  Hsp47 binds transiently to collagen types I to IV and avidly to denatured collagen substrates; thus, its role in procollagen processing and transport seems firmly established.	bind
23545	5	6805	5	13	NULL	NULL	NULL	Hsp47	GP		bind		avidly			collagen substrates	GP	denatured			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_219	9686751	176  Hsp47 binds transiently to collagen types I to IV and avidly to denatured collagen substrates; thus, its role in procollagen processing and transport seems firmly established.	bind
23546	6	6805	5	13	NULL	NULL	NULL	Hsp47	GP		plays a role in					procollagen	GP	 processing of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_219	9686751	176  Hsp47 binds transiently to collagen types I to IV and avidly to denatured collagen substrates; thus, its role in procollagen processing and transport seems firmly established.	bind
23547	7	6805	5	13	NULL	NULL	NULL	Hsp47	GP		plays a role in					procollagen 	GP	transport of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_219	9686751	176  Hsp47 binds transiently to collagen types I to IV and avidly to denatured collagen substrates; thus, its role in procollagen processing and transport seems firmly established.	bind
19723	1	6805	6	NULL	NULL	0	NULL	Hsp47	NULL		bind	NULL	transiently			collagen type I	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_219	9686751	176  Hsp47 binds transiently to collagen types I to IV and avidly to denatured collagen substrates; thus, its role in procollagen processing and transport seems firmly established.	bind
19724	2	6805	6	NULL	NULL	0	NULL	Hsp47	NULL		bind	NULL	transiently			collagen type IV	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_219	9686751	176  Hsp47 binds transiently to collagen types I to IV and avidly to denatured collagen substrates; thus, its role in procollagen processing and transport seems firmly established.	bind
19725	3	6805	6	NULL	NULL	0	NULL	Hsp47	NULL		bind	NULL	avidly			collagen substrates	NULL	denatured			NULL		0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_219	9686751	176  Hsp47 binds transiently to collagen types I to IV and avidly to denatured collagen substrates; thus, its role in procollagen processing and transport seems firmly established.	bind
19726	4	6805	6	10	NULL	0	NULL	Hsp47			plays a role in					procollagen 		processing of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_219	9686751	176  Hsp47 binds transiently to collagen types I to IV and avidly to denatured collagen substrates; thus, its role in procollagen processing and transport seems firmly established.	bind
19727	5	6805	6	10	NULL	0	NULL	Hsp47			plays a role in					procollagen		 transport of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_219	9686751	176  Hsp47 binds transiently to collagen types I to IV and avidly to denatured collagen substrates; thus, its role in procollagen processing and transport seems firmly established.	bind
56591	6	6805	6	10	NULL	0	NULL	Hsp47			bind		transiently			collagen type II					NULL		0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_219	9686751	176  Hsp47 binds transiently to collagen types I to IV and avidly to denatured collagen substrates; thus, its role in procollagen processing and transport seems firmly established.	bind
56592	7	6805	6	10	NULL	0	NULL	Hsp47			bind		transiently			collagen type III					NULL		0	NULL	NULL	NULL	gw60_circulationres_83_2_117_s_219	9686751	176  Hsp47 binds transiently to collagen types I to IV and avidly to denatured collagen substrates; thus, its role in procollagen processing and transport seems firmly established.	bind
23548	1	6806	5	13	NULL	NULL	NULL	TRL	GP		bind					macrophage membrane-binding proteins	GP	specific			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2474_s_230	10521378	177 178  This effect may be due to apoE-independent binding of TRL to specific macrophage membrane-binding proteins 179 180  or may be the result of cellular recognition and uptake of oxidized remnant lipoproteins.	bind
23549	2	6806	5	13	NULL	NULL	NULL	statement 1	Process		is independent of					apoE	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2474_s_230	10521378	177 178  This effect may be due to apoE-independent binding of TRL to specific macrophage membrane-binding proteins 179 180  or may be the result of cellular recognition and uptake of oxidized remnant lipoproteins.	bind
19728	1	6806	6	NULL	NULL	0	NULL	TRL	NULL		bind	NULL				macrophage membrane-binding proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2474_s_230	10521378	177 178  This effect may be due to apoE-independent binding of TRL to specific macrophage membrane-binding proteins 179 180  or may be the result of cellular recognition and uptake of oxidized remnant lipoproteins.	bind
19729	2	6806	6	NULL	NULL	0	NULL	statement 1	NULL		is independent of	NULL				apoE	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2474_s_230	10521378	177 178  This effect may be due to apoE-independent binding of TRL to specific macrophage membrane-binding proteins 179 180  or may be the result of cellular recognition and uptake of oxidized remnant lipoproteins.	bind
23550	1	6807	5	13	NULL	NULL	NULL	mAKAP	GP		bind					PKA	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_99_8_816_s_183	17038651	178 This latter complex is interesting because mAKAP not only binds PKA and PDE4D3 but also Epac1 and extracellular signal-regulated kinase 5 (ERK5).	bind
23551	2	6807	5	13	NULL	NULL	NULL	mAKAP	GP		bind					PDE4D3	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_99_8_816_s_183	17038651	178 This latter complex is interesting because mAKAP not only binds PKA and PDE4D3 but also Epac1 and extracellular signal-regulated kinase 5 (ERK5).	bind
23552	3	6807	5	13	NULL	NULL	NULL	mAKAP	GP		bind					Epac1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_99_8_816_s_183	17038651	178 This latter complex is interesting because mAKAP not only binds PKA and PDE4D3 but also Epac1 and extracellular signal-regulated kinase 5 (ERK5).	bind
23553	4	6807	5	13	NULL	NULL	NULL	mAKAP	GP		bind					ERK5	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_99_8_816_s_183	17038651	178 This latter complex is interesting because mAKAP not only binds PKA and PDE4D3 but also Epac1 and extracellular signal-regulated kinase 5 (ERK5).	bind
23554	5	6807	5	13	NULL	NULL	NULL	ERK5	GP		is					extracellular signal-regulated kinase 5	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_99_8_816_s_183	17038651	178 This latter complex is interesting because mAKAP not only binds PKA and PDE4D3 but also Epac1 and extracellular signal-regulated kinase 5 (ERK5).	bind
19730	1	6807	6	NULL	NULL	0	NULL	mAKAP	NULL		bind	NULL				PKA	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_99_8_816_s_183	17038651	178 This latter complex is interesting because mAKAP not only binds PKA and PDE4D3 but also Epac1 and extracellular signal-regulated kinase 5 (ERK5).	bind
19731	2	6807	6	NULL	NULL	0	NULL	mAKAP	NULL		bind	NULL				PDE4D3	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_99_8_816_s_183	17038651	178 This latter complex is interesting because mAKAP not only binds PKA and PDE4D3 but also Epac1 and extracellular signal-regulated kinase 5 (ERK5).	bind
19732	3	6807	6	NULL	NULL	0	NULL	mAKAP	NULL		bind	NULL				Epac1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_99_8_816_s_183	17038651	178 This latter complex is interesting because mAKAP not only binds PKA and PDE4D3 but also Epac1 and extracellular signal-regulated kinase 5 (ERK5).	bind
19733	4	6807	6	NULL	NULL	0	NULL	mAKAP	NULL		bind	NULL				ERK5	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_99_8_816_s_183	17038651	178 This latter complex is interesting because mAKAP not only binds PKA and PDE4D3 but also Epac1 and extracellular signal-regulated kinase 5 (ERK5).	bind
19734	5	6807	6	NULL	NULL	0	NULL	ERK5	NULL		is	NULL				extracellular signal-regulated kinase 5	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_99_8_816_s_183	17038651	178 This latter complex is interesting because mAKAP not only binds PKA and PDE4D3 but also Epac1 and extracellular signal-regulated kinase 5 (ERK5).	bind
23627	1	6808	5	13	NULL	NULL	NULL	ER	GP		bind					PI-9	GP			ERU	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_6_5025_s_167	14617632	17beta -Estradiol and Moxestrol Induce Similar Binding of ER to the PI-9 ERU and to the pS2 ERE --	bind
23628	2	6808	5	13	NULL	NULL	NULL	ER	GP		bind					pS2	GP			ERE	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_6_5025_s_167	14617632	17beta -Estradiol and Moxestrol Induce Similar Binding of ER to the PI-9 ERU and to the pS2 ERE --	bind
19735	1	6808	6	10	NULL	0	NULL	ER			bind					PI-9 				ERU	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_6_5025_s_167	14617632	17beta -Estradiol and Moxestrol Induce Similar Binding of ER to the PI-9 ERU and to the pS2 ERE --	bind
19736	2	6808	6	NULL	NULL	0	NULL	ER	NULL		bind	NULL				pS2	NULL			ERE	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_6_5025_s_167	14617632	17beta -Estradiol and Moxestrol Induce Similar Binding of ER to the PI-9 ERU and to the pS2 ERE --	bind
23639	1	6809	5	13	NULL	NULL	NULL	Ah receptor complex	GP		bind									AhRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_6_3430_s_254	9920887	17beta-Estradiol reduced Ah receptor complex binding to AhRE. ECC-1 cells were exposed to TCDD ( T) (10 nM) and 17beta-estradiol ( E2) (10 nM) alone or in combination, or with solvent alone (0.1% Me2SO ( DMSO)), for 1 h, after which nuclear protein extracts were prepared.	bind
23640	2	6809	5	13	NULL	NULL	NULL	17beta-Estradiol	Chemical		reduces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_6_3430_s_254	9920887	17beta-Estradiol reduced Ah receptor complex binding to AhRE. ECC-1 cells were exposed to TCDD ( T) (10 nM) and 17beta-estradiol ( E2) (10 nM) alone or in combination, or with solvent alone (0.1% Me2SO ( DMSO)), for 1 h, after which nuclear protein extracts were prepared.	bind
19737	1	6809	6	NULL	NULL	0	NULL	Ah receptor complex	NULL		bind	NULL					NULL			AhRE	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_6_3430_s_254	9920887	17beta-Estradiol reduced Ah receptor complex binding to AhRE. ECC-1 cells were exposed to TCDD ( T) (10 nM) and 17beta-estradiol ( E2) (10 nM) alone or in combination, or with solvent alone (0.1% Me2SO ( DMSO)), for 1 h, after which nuclear protein extracts were prepared.	bind
19738	2	6809	6	NULL	NULL	0	NULL	17beta-Estradiol	NULL		reduces	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_6_3430_s_254	9920887	17beta-Estradiol reduced Ah receptor complex binding to AhRE. ECC-1 cells were exposed to TCDD ( T) (10 nM) and 17beta-estradiol ( E2) (10 nM) alone or in combination, or with solvent alone (0.1% Me2SO ( DMSO)), for 1 h, after which nuclear protein extracts were prepared.	bind
23652	1	6811	5	13	NULL	NULL	NULL	binuclear zinc AlcR activator	GP		bind		specifically			DNA	NucleicAcid				NULL	in Aspergillus nidulans	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_10_2181_s_247	11353088	18       Nikolaev,I., Lenouvel,F. and Felenbok,B. (1999) Unique DNA binding specificity of the binuclear zinc AlcR activator of the ethanol utilization pathway in  Aspergillus nidulans.	bind
44701	2	6811	5	13	NULL	NULL	NULL	binuclear zinc AlcR activator	GP		belongs to					ethanol utilization pathway	Process				NULL	Aspergillus nidulans	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_10_2181_s_247	11353088	18       Nikolaev,I., Lenouvel,F. and Felenbok,B. (1999) Unique DNA binding specificity of the binuclear zinc AlcR activator of the ethanol utilization pathway in  Aspergillus nidulans.	bind
19739	1	6811	6	10	NULL	0	NULL	binuclear zinc AlcR activator 			bind					DNA					NULL	Aspergillus nidulans	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_10_2181_s_247	11353088	18       Nikolaev,I., Lenouvel,F. and Felenbok,B. (1999) Unique DNA binding specificity of the binuclear zinc AlcR activator of the ethanol utilization pathway in  Aspergillus nidulans.	bind
56593	2	6811	6	10	NULL	0	NULL	binuclear zinc AlcR activator			belongs to					ethanol utilization pathway					NULL	Aspergillus nidulans	0	NULL	NULL	NULL	gw60_nucleicacidsres_29_10_2181_s_247	11353088	18       Nikolaev,I., Lenouvel,F. and Felenbok,B. (1999) Unique DNA binding specificity of the binuclear zinc AlcR activator of the ethanol utilization pathway in  Aspergillus nidulans.	bind
23658	1	6813	5	13	NULL	NULL	NULL	DNA	NucleicAcid	nucleosomal	regulates					Hat1 acetyltransferase	GP	human	core-histone-binding subunit		NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_15_3131_s_239	11470869	18       Verreault,A., Kaufman,P.D., Kobayashi,R. and Stillman,B. (1998) Nucleosomal DNA regulates the core-histone-binding subunit of the human Hat1 acetyltransferase.	bind
19740	1	6813	6	10	NULL	0	NULL	 DNA		Nucleosomal	regulates					Hat1 acetyltransferase		human	core-histone-binding subunit		NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_15_3131_s_239	11470869	18       Verreault,A., Kaufman,P.D., Kobayashi,R. and Stillman,B. (1998) Nucleosomal DNA regulates the core-histone-binding subunit of the human Hat1 acetyltransferase.	bind
23675	1	6814	5	13	NULL	NULL	NULL	Megalin/gp330	GP		bind					plasminogen	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_552_s_248	10073957	18  19 20 21 22 23 24 25  Megalin/gp330 is known to be the only member of the  LDLR gene family to bind the apo(a) homologue plasminogen, 33 36  thus suggesting that Lp(a) might bind to megalin/gp330 by either apoB100, apo(a), or both apolipoproteins.	bind
23678	2	6814	5	13	NULL	NULL	NULL	Lp(a)	GP		bind		might			megalin/gp330	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_552_s_248	10073957	18  19 20 21 22 23 24 25  Megalin/gp330 is known to be the only member of the  LDLR gene family to bind the apo(a) homologue plasminogen, 33 36  thus suggesting that Lp(a) might bind to megalin/gp330 by either apoB100, apo(a), or both apolipoproteins.	bind
23681	3	6814	5	13	NULL	NULL	NULL	statement 2	Process		occurs by					apoB100	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_552_s_248	10073957	18  19 20 21 22 23 24 25  Megalin/gp330 is known to be the only member of the  LDLR gene family to bind the apo(a) homologue plasminogen, 33 36  thus suggesting that Lp(a) might bind to megalin/gp330 by either apoB100, apo(a), or both apolipoproteins.	bind
23682	4	6814	5	13	NULL	NULL	NULL	statement 2	Process		occurs by					apo(a)	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_552_s_248	10073957	18  19 20 21 22 23 24 25  Megalin/gp330 is known to be the only member of the  LDLR gene family to bind the apo(a) homologue plasminogen, 33 36  thus suggesting that Lp(a) might bind to megalin/gp330 by either apoB100, apo(a), or both apolipoproteins.	bind
23684	5	6814	5	13	NULL	NULL	NULL	statement 3	Process		occurs simulataneous with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_552_s_248	10073957	18  19 20 21 22 23 24 25  Megalin/gp330 is known to be the only member of the  LDLR gene family to bind the apo(a) homologue plasminogen, 33 36  thus suggesting that Lp(a) might bind to megalin/gp330 by either apoB100, apo(a), or both apolipoproteins.	bind
23685	6	6814	5	13	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_552_s_248	10073957	18  19 20 21 22 23 24 25  Megalin/gp330 is known to be the only member of the  LDLR gene family to bind the apo(a) homologue plasminogen, 33 36  thus suggesting that Lp(a) might bind to megalin/gp330 by either apoB100, apo(a), or both apolipoproteins.	bind
23687	7	6814	5	13	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_552_s_248	10073957	18  19 20 21 22 23 24 25  Megalin/gp330 is known to be the only member of the  LDLR gene family to bind the apo(a) homologue plasminogen, 33 36  thus suggesting that Lp(a) might bind to megalin/gp330 by either apoB100, apo(a), or both apolipoproteins.	bind
56594	8	6814	5	13	NULL	NULL	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_552_s_248	10073957	18  19 20 21 22 23 24 25  Megalin/gp330 is known to be the only member of the  LDLR gene family to bind the apo(a) homologue plasminogen, 33 36  thus suggesting that Lp(a) might bind to megalin/gp330 by either apoB100, apo(a), or both apolipoproteins.	bind
56595	9	6814	5	13	NULL	NULL	NULL	Megalin/gp330	GP		is a member of					LDLR gene family	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_552_s_248	10073957	18  19 20 21 22 23 24 25  Megalin/gp330 is known to be the only member of the  LDLR gene family to bind the apo(a) homologue plasminogen, 33 36  thus suggesting that Lp(a) might bind to megalin/gp330 by either apoB100, apo(a), or both apolipoproteins.	bind
56596	10	6814	5	13	NULL	NULL	NULL	plasminogen	GP		is homologous to					apo(a) 	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_552_s_248	10073957	18  19 20 21 22 23 24 25  Megalin/gp330 is known to be the only member of the  LDLR gene family to bind the apo(a) homologue plasminogen, 33 36  thus suggesting that Lp(a) might bind to megalin/gp330 by either apoB100, apo(a), or both apolipoproteins.	bind
19741	1	6814	6	10	NULL	0	NULL	Megalin/gp330			bind					 plasminogen					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_552_s_248	10073957	18  19 20 21 22 23 24 25  Megalin/gp330 is known to be the only member of the  LDLR gene family to bind the apo(a) homologue plasminogen, 33 36  thus suggesting that Lp(a) might bind to megalin/gp330 by either apoB100, apo(a), or both apolipoproteins.	bind
19742	2	6814	6	NULL	NULL	0	NULL	Megalin/gp330	NULL		is a member of	NULL				LDLR gene family	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_552_s_248	10073957	18  19 20 21 22 23 24 25  Megalin/gp330 is known to be the only member of the  LDLR gene family to bind the apo(a) homologue plasminogen, 33 36  thus suggesting that Lp(a) might bind to megalin/gp330 by either apoB100, apo(a), or both apolipoproteins.	bind
19743	3	6814	6	NULL	NULL	0	NULL	Lp(a)	NULL		bind	NULL	may			megalin/gp330	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_552_s_248	10073957	18  19 20 21 22 23 24 25  Megalin/gp330 is known to be the only member of the  LDLR gene family to bind the apo(a) homologue plasminogen, 33 36  thus suggesting that Lp(a) might bind to megalin/gp330 by either apoB100, apo(a), or both apolipoproteins.	bind
19744	4	6814	6	NULL	NULL	0	NULL	statement 3	NULL		occurs by	NULL				apoB100	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_552_s_248	10073957	18  19 20 21 22 23 24 25  Megalin/gp330 is known to be the only member of the  LDLR gene family to bind the apo(a) homologue plasminogen, 33 36  thus suggesting that Lp(a) might bind to megalin/gp330 by either apoB100, apo(a), or both apolipoproteins.	bind
19745	5	6814	6	NULL	NULL	0	NULL	statement 3	NULL		occurs by	NULL				apo(a)	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_552_s_248	10073957	18  19 20 21 22 23 24 25  Megalin/gp330 is known to be the only member of the  LDLR gene family to bind the apo(a) homologue plasminogen, 33 36  thus suggesting that Lp(a) might bind to megalin/gp330 by either apoB100, apo(a), or both apolipoproteins.	bind
19746	6	6814	6	NULL	NULL	0	NULL	statement 4	NULL		is an alternative to	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_552_s_248	10073957	18  19 20 21 22 23 24 25  Megalin/gp330 is known to be the only member of the  LDLR gene family to bind the apo(a) homologue plasminogen, 33 36  thus suggesting that Lp(a) might bind to megalin/gp330 by either apoB100, apo(a), or both apolipoproteins.	bind
56597	7	6814	6	10	NULL	0	NULL	statement 4			occur simulataneous with					statement 5					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_552_s_248	10073957	18  19 20 21 22 23 24 25  Megalin/gp330 is known to be the only member of the  LDLR gene family to bind the apo(a) homologue plasminogen, 33 36  thus suggesting that Lp(a) might bind to megalin/gp330 by either apoB100, apo(a), or both apolipoproteins.	bind
56598	8	6814	6	10	NULL	0	NULL	statement 4			is an alternative to					statement 7					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_552_s_248	10073957	18  19 20 21 22 23 24 25  Megalin/gp330 is known to be the only member of the  LDLR gene family to bind the apo(a) homologue plasminogen, 33 36  thus suggesting that Lp(a) might bind to megalin/gp330 by either apoB100, apo(a), or both apolipoproteins.	bind
56599	9	6814	6	10	NULL	0	NULL	statement 5			is an alternative to					statement 7					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_552_s_248	10073957	18  19 20 21 22 23 24 25  Megalin/gp330 is known to be the only member of the  LDLR gene family to bind the apo(a) homologue plasminogen, 33 36  thus suggesting that Lp(a) might bind to megalin/gp330 by either apoB100, apo(a), or both apolipoproteins.	bind
56600	10	6814	6	10	NULL	0	NULL	plasminogen			is homologous to					apo(a) 					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_552_s_248	10073957	18  19 20 21 22 23 24 25  Megalin/gp330 is known to be the only member of the  LDLR gene family to bind the apo(a) homologue plasminogen, 33 36  thus suggesting that Lp(a) might bind to megalin/gp330 by either apoB100, apo(a), or both apolipoproteins.	bind
23719	1	6815	5	13	NULL	NULL	NULL	TSP1	GP		bind					TGF-beta1	GP	latent			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_4_1255_s_33	11583953	18  Based on the identified interaction sites between TSP1 and TGF-beta1 it has been suggested that TSP1 and TSP2 may compete for binding to latent TGF-beta1, but only binding of TSP1 would lead to its activation.	bind
23720	2	6815	5	13	NULL	NULL	NULL	TSP2	GP		bind					TGF-beta1	GP	latent			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_4_1255_s_33	11583953	18  Based on the identified interaction sites between TSP1 and TGF-beta1 it has been suggested that TSP1 and TSP2 may compete for binding to latent TGF-beta1, but only binding of TSP1 would lead to its activation.	bind
23721	3	6815	5	13	NULL	NULL	NULL	statement 1	Process		competes with		may			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_4_1255_s_33	11583953	18  Based on the identified interaction sites between TSP1 and TGF-beta1 it has been suggested that TSP1 and TSP2 may compete for binding to latent TGF-beta1, but only binding of TSP1 would lead to its activation.	bind
23722	4	6815	5	13	NULL	NULL	NULL	statement 1	Process		leads to					TGF-beta1	GP	activation of latent			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_4_1255_s_33	11583953	18  Based on the identified interaction sites between TSP1 and TGF-beta1 it has been suggested that TSP1 and TSP2 may compete for binding to latent TGF-beta1, but only binding of TSP1 would lead to its activation.	bind
19747	1	6815	6	NULL	NULL	0	NULL	TSP1	NULL		bind	NULL				TGF-beta1	NULL	latent			NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_4_1255_s_33	11583953	18  Based on the identified interaction sites between TSP1 and TGF-beta1 it has been suggested that TSP1 and TSP2 may compete for binding to latent TGF-beta1, but only binding of TSP1 would lead to its activation.	bind
19748	2	6815	6	NULL	NULL	0	NULL	TSP2	NULL		bind	NULL				TGF-beta1	NULL	latent			NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_4_1255_s_33	11583953	18  Based on the identified interaction sites between TSP1 and TGF-beta1 it has been suggested that TSP1 and TSP2 may compete for binding to latent TGF-beta1, but only binding of TSP1 would lead to its activation.	bind
19749	3	6815	6	NULL	NULL	0	NULL	statement 1	NULL		competes	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_4_1255_s_33	11583953	18  Based on the identified interaction sites between TSP1 and TGF-beta1 it has been suggested that TSP1 and TSP2 may compete for binding to latent TGF-beta1, but only binding of TSP1 would lead to its activation.	bind
19750	4	6815	6	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				TGF-beta1	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_4_1255_s_33	11583953	18  Based on the identified interaction sites between TSP1 and TGF-beta1 it has been suggested that TSP1 and TSP2 may compete for binding to latent TGF-beta1, but only binding of TSP1 would lead to its activation.	bind
23723	1	6816	5	13	NULL	NULL	NULL				lowers		greatly	Tyr-13 point mutations		monocyte chemoattractant protein-1 receptor	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_2_591_s_28	10433951	18  Consistent with the concept that tyrosine is important in binding to receptor, point mutations of Tyr-13 greatly lowered monocyte chemoattractant protein-1 receptor binding and activity, 19 and changing Tyr-28 to aspartate essentially abolished the monocyte chemoattractant activity of monocyte chemoattractant protein-1.	bind
23724	3	6816	5	10	NULL	0	NULL				is changed to			Tyr-28					aspartate		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_2_591_s_28	10433951	18  Consistent with the concept that tyrosine is important in binding to receptor, point mutations of Tyr-13 greatly lowered monocyte chemoattractant protein-1 receptor binding and activity, 19 and changing Tyr-28 to aspartate essentially abolished the monocyte chemoattractant activity of monocyte chemoattractant protein-1.	bind
23725	5	6816	5	13	NULL	NULL	NULL	statement 3	Process		abolishes					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_2_591_s_28	10433951	18  Consistent with the concept that tyrosine is important in binding to receptor, point mutations of Tyr-13 greatly lowered monocyte chemoattractant protein-1 receptor binding and activity, 19 and changing Tyr-28 to aspartate essentially abolished the monocyte chemoattractant activity of monocyte chemoattractant protein-1.	bind
23728	2	6816	5	13	NULL	NULL	NULL				lowers		greatly	Tyr-13 point mutations		monocyte chemoattractant protein-1 receptor	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_2_591_s_28	10433951	18  Consistent with the concept that tyrosine is important in binding to receptor, point mutations of Tyr-13 greatly lowered monocyte chemoattractant protein-1 receptor binding and activity, 19 and changing Tyr-28 to aspartate essentially abolished the monocyte chemoattractant activity of monocyte chemoattractant protein-1.	bind
58592	4	6816	5	13	NULL	NULL	NULL	monocyte chemoattractant protein-1	GP		activates					monocyte chemoattractant	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_2_591_s_28	10433951	18  Consistent with the concept that tyrosine is important in binding to receptor, point mutations of Tyr-13 greatly lowered monocyte chemoattractant protein-1 receptor binding and activity, 19 and changing Tyr-28 to aspartate essentially abolished the monocyte chemoattractant activity of monocyte chemoattractant protein-1.	bind
19854	1	6816	6	10	NULL	0	NULL				lowers		greatly	Tyr-13 point mutations		monocyte chemoattractant protein-1 receptor		binding of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_2_591_s_28	10433951	18  Consistent with the concept that tyrosine is important in binding to receptor, point mutations of Tyr-13 greatly lowered monocyte chemoattractant protein-1 receptor binding and activity, 19 and changing Tyr-28 to aspartate essentially abolished the monocyte chemoattractant activity of monocyte chemoattractant protein-1.	bind
19855	2	6816	6	10	NULL	0	NULL				lowers		greatly	Tyr-13 point mutations		monocyte chemoattractant protein-1 receptor		activity of 			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_2_591_s_28	10433951	18  Consistent with the concept that tyrosine is important in binding to receptor, point mutations of Tyr-13 greatly lowered monocyte chemoattractant protein-1 receptor binding and activity, 19 and changing Tyr-28 to aspartate essentially abolished the monocyte chemoattractant activity of monocyte chemoattractant protein-1.	bind
19856	3	6816	6	NULL	NULL	0	NULL		NULL		is changed to	NULL		Tyr-28			NULL		Aspartate		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_2_591_s_28	10433951	18  Consistent with the concept that tyrosine is important in binding to receptor, point mutations of Tyr-13 greatly lowered monocyte chemoattractant protein-1 receptor binding and activity, 19 and changing Tyr-28 to aspartate essentially abolished the monocyte chemoattractant activity of monocyte chemoattractant protein-1.	bind
19857	4	6816	6	10	NULL	0	NULL	monocyte chemoattractant protein-1			activates					monocyte chemoattractant					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_2_591_s_28	10433951	18  Consistent with the concept that tyrosine is important in binding to receptor, point mutations of Tyr-13 greatly lowered monocyte chemoattractant protein-1 receptor binding and activity, 19 and changing Tyr-28 to aspartate essentially abolished the monocyte chemoattractant activity of monocyte chemoattractant protein-1.	bind
19858	5	6816	6	NULL	NULL	0	NULL	statement 3	NULL		abolishes	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_2_591_s_28	10433951	18  Consistent with the concept that tyrosine is important in binding to receptor, point mutations of Tyr-13 greatly lowered monocyte chemoattractant protein-1 receptor binding and activity, 19 and changing Tyr-28 to aspartate essentially abolished the monocyte chemoattractant activity of monocyte chemoattractant protein-1.	bind
23726	1	6817	5	13	NULL	NULL	NULL			point mutations of	lowered		greatly	Tyr-13		monocyte chemoattractant protein-1 receptor	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_2_591_s_227	10433951	18  Consistent with the concept that tyrosine is important in binding to receptor, Steitz et al 19  reported that point mutations of Tyr-13 greatly lowered monocyte chemoattractant protein-1 receptor binding and activity.	bind
23727	2	6817	5	13	NULL	NULL	NULL			point mutations of	lowered		greatly	Tyr-13		monocyte chemoattractant protein-1 receptor	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_2_591_s_227	10433951	18  Consistent with the concept that tyrosine is important in binding to receptor, Steitz et al 19  reported that point mutations of Tyr-13 greatly lowered monocyte chemoattractant protein-1 receptor binding and activity.	bind
19760	1	6817	6	13	NULL	NULL	NULL	tyrosine	AminoAcid		is important for					receptor	GP	binding to			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_2_591_s_227	10433951	18  Consistent with the concept that tyrosine is important in binding to receptor, Steitz et al 19  reported that point mutations of Tyr-13 greatly lowered monocyte chemoattractant protein-1 receptor binding and activity.	bind
19761	2	6817	6	NULL	NULL	0	NULL		NULL	point mutation	lowered	NULL		Tyr-13		monocyte chemoattractant protein-1 receptor	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_2_591_s_227	10433951	18  Consistent with the concept that tyrosine is important in binding to receptor, Steitz et al 19  reported that point mutations of Tyr-13 greatly lowered monocyte chemoattractant protein-1 receptor binding and activity.	bind
19762	3	6817	6	NULL	NULL	0	NULL		NULL	point mutation	lowered	NULL		Tyr-13		monocyte chemoattractant protein-1 receptor	NULL	activity of 			NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_2_591_s_227	10433951	18  Consistent with the concept that tyrosine is important in binding to receptor, Steitz et al 19  reported that point mutations of Tyr-13 greatly lowered monocyte chemoattractant protein-1 receptor binding and activity.	bind
23729	1	6818	5	13	NULL	NULL	NULL	FN	GP		bind					ECs	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1544_s_154	8977460	18  Furthermore, heparin failed to inhibit binding of FN to ECs (Fig 8B  ), even though concentration-dependent binding of FN to ECs was demonstrated (Fig 8A  ).	bind
23730	2	6818	5	13	NULL	NULL	NULL	heparin	Chemical		does not inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1544_s_154	8977460	18  Furthermore, heparin failed to inhibit binding of FN to ECs (Fig 8B  ), even though concentration-dependent binding of FN to ECs was demonstrated (Fig 8A  ).	bind
44702	3	6818	5	13	NULL	NULL	NULL	statement 1	Process		depends on					concentration	QuantityOrMeasure				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1544_s_154	8977460	18  Furthermore, heparin failed to inhibit binding of FN to ECs (Fig 8B  ), even though concentration-dependent binding of FN to ECs was demonstrated (Fig 8A  ).	bind
19763	1	6818	6	NULL	NULL	0	NULL	FN	NULL		bind	NULL				EC	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1544_s_154	8977460	18  Furthermore, heparin failed to inhibit binding of FN to ECs (Fig 8B  ), even though concentration-dependent binding of FN to ECs was demonstrated (Fig 8A  ).	bind
19764	2	6818	6	NULL	NULL	0	NULL	heparin	NULL		does not inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1544_s_154	8977460	18  Furthermore, heparin failed to inhibit binding of FN to ECs (Fig 8B  ), even though concentration-dependent binding of FN to ECs was demonstrated (Fig 8A  ).	bind
19766	3	6818	6	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				concentration	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1544_s_154	8977460	18  Furthermore, heparin failed to inhibit binding of FN to ECs (Fig 8B  ), even though concentration-dependent binding of FN to ECs was demonstrated (Fig 8A  ).	bind
23731	1	6819	5	13	NULL	NULL	NULL	antibodies	GP		bind		specifically			gelB	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_303_s_218	10880400	18  In the studies of Lelongt et al, 8  the antibodies and TIMP-1 which bind specifically to gelB may somehow, either directly or indirectly, disrupt cell-cell or cell-matrix interactions that are necessary for branching morphogenesis.	bind
23732	2	6819	5	13	NULL	NULL	NULL	TIMP-1	GP		bind		specifically			gelB	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_303_s_218	10880400	18  In the studies of Lelongt et al, 8  the antibodies and TIMP-1 which bind specifically to gelB may somehow, either directly or indirectly, disrupt cell-cell or cell-matrix interactions that are necessary for branching morphogenesis.	bind
23733	3	6819	5	13	NULL	NULL	NULL	statement 1	Process		disrupt		directly			cell-cell interactions	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_303_s_218	10880400	18  In the studies of Lelongt et al, 8  the antibodies and TIMP-1 which bind specifically to gelB may somehow, either directly or indirectly, disrupt cell-cell or cell-matrix interactions that are necessary for branching morphogenesis.	bind
23734	4	6819	5	13	NULL	NULL	NULL	statement 1	Process		disrupt		indirectly			cell-cell interactions	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_303_s_218	10880400	18  In the studies of Lelongt et al, 8  the antibodies and TIMP-1 which bind specifically to gelB may somehow, either directly or indirectly, disrupt cell-cell or cell-matrix interactions that are necessary for branching morphogenesis.	bind
23735	5	6819	5	13	NULL	NULL	NULL	statement 2	Process		disrupt		directly			cell-cell interactions	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_303_s_218	10880400	18  In the studies of Lelongt et al, 8  the antibodies and TIMP-1 which bind specifically to gelB may somehow, either directly or indirectly, disrupt cell-cell or cell-matrix interactions that are necessary for branching morphogenesis.	bind
23736	6	6819	5	13	NULL	NULL	NULL	statement 2	Process		disrupt		indirectly			cell-cell interactions	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_303_s_218	10880400	18  In the studies of Lelongt et al, 8  the antibodies and TIMP-1 which bind specifically to gelB may somehow, either directly or indirectly, disrupt cell-cell or cell-matrix interactions that are necessary for branching morphogenesis.	bind
23737	7	6819	5	13	NULL	NULL	NULL	statement 1	Process		disrupt		directly			cell-matrix interactions	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_303_s_218	10880400	18  In the studies of Lelongt et al, 8  the antibodies and TIMP-1 which bind specifically to gelB may somehow, either directly or indirectly, disrupt cell-cell or cell-matrix interactions that are necessary for branching morphogenesis.	bind
23738	8	6819	5	13	NULL	NULL	NULL	statement 1	Process		disrupt		indirectly			cell-matrix interactions	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_303_s_218	10880400	18  In the studies of Lelongt et al, 8  the antibodies and TIMP-1 which bind specifically to gelB may somehow, either directly or indirectly, disrupt cell-cell or cell-matrix interactions that are necessary for branching morphogenesis.	bind
23739	9	6819	5	13	NULL	NULL	NULL	statement 2	Process		disrupt		directly			cell-matrix interactions	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_303_s_218	10880400	18  In the studies of Lelongt et al, 8  the antibodies and TIMP-1 which bind specifically to gelB may somehow, either directly or indirectly, disrupt cell-cell or cell-matrix interactions that are necessary for branching morphogenesis.	bind
23740	10	6819	5	13	NULL	NULL	NULL	statement 2	Process		disrupt		indirectly			cell-matrix interactions	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_303_s_218	10880400	18  In the studies of Lelongt et al, 8  the antibodies and TIMP-1 which bind specifically to gelB may somehow, either directly or indirectly, disrupt cell-cell or cell-matrix interactions that are necessary for branching morphogenesis.	bind
23741	11	6819	5	13	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_303_s_218	10880400	18  In the studies of Lelongt et al, 8  the antibodies and TIMP-1 which bind specifically to gelB may somehow, either directly or indirectly, disrupt cell-cell or cell-matrix interactions that are necessary for branching morphogenesis.	bind
23742	12	6819	5	13	NULL	NULL	NULL	statement 5	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_303_s_218	10880400	18  In the studies of Lelongt et al, 8  the antibodies and TIMP-1 which bind specifically to gelB may somehow, either directly or indirectly, disrupt cell-cell or cell-matrix interactions that are necessary for branching morphogenesis.	bind
23743	13	6819	5	13	NULL	NULL	NULL	statement 7	Process		is an alternative to					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_303_s_218	10880400	18  In the studies of Lelongt et al, 8  the antibodies and TIMP-1 which bind specifically to gelB may somehow, either directly or indirectly, disrupt cell-cell or cell-matrix interactions that are necessary for branching morphogenesis.	bind
23744	14	6819	5	13	NULL	NULL	NULL	statement 9	Process		is an alternative to					statement 10	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_303_s_218	10880400	18  In the studies of Lelongt et al, 8  the antibodies and TIMP-1 which bind specifically to gelB may somehow, either directly or indirectly, disrupt cell-cell or cell-matrix interactions that are necessary for branching morphogenesis.	bind
56603	15	6819	5	13	NULL	NULL	NULL	cell-cell interactions	Process		are necessary for					branching morphogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_303_s_218	10880400	18  In the studies of Lelongt et al, 8  the antibodies and TIMP-1 which bind specifically to gelB may somehow, either directly or indirectly, disrupt cell-cell or cell-matrix interactions that are necessary for branching morphogenesis.	bind
56604	16	6819	5	13	NULL	NULL	NULL	cell-matrix interactions	Process		are necessary for					branching morphogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_303_s_218	10880400	18  In the studies of Lelongt et al, 8  the antibodies and TIMP-1 which bind specifically to gelB may somehow, either directly or indirectly, disrupt cell-cell or cell-matrix interactions that are necessary for branching morphogenesis.	bind
19767	1	6819	6	NULL	NULL	0	NULL	antibodies	NULL		bind	NULL	specifically			gelB	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_1_303_s_218	10880400	18  In the studies of Lelongt et al, 8  the antibodies and TIMP-1 which bind specifically to gelB may somehow, either directly or indirectly, disrupt cell-cell or cell-matrix interactions that are necessary for branching morphogenesis.	bind
19768	2	6819	6	NULL	NULL	0	NULL	TIMP-1	NULL		bind	NULL	specifically			gelB	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_1_303_s_218	10880400	18  In the studies of Lelongt et al, 8  the antibodies and TIMP-1 which bind specifically to gelB may somehow, either directly or indirectly, disrupt cell-cell or cell-matrix interactions that are necessary for branching morphogenesis.	bind
19769	3	6819	6	NULL	NULL	0	NULL	cell-cell interactions	NULL		are necessary for	NULL				branching morphogenesis	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_1_303_s_218	10880400	18  In the studies of Lelongt et al, 8  the antibodies and TIMP-1 which bind specifically to gelB may somehow, either directly or indirectly, disrupt cell-cell or cell-matrix interactions that are necessary for branching morphogenesis.	bind
19770	4	6819	6	NULL	NULL	0	NULL	cell-matrix interactions	NULL		are necessary for	NULL				branching morphogenesis	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_1_303_s_218	10880400	18  In the studies of Lelongt et al, 8  the antibodies and TIMP-1 which bind specifically to gelB may somehow, either directly or indirectly, disrupt cell-cell or cell-matrix interactions that are necessary for branching morphogenesis.	bind
19771	5	6819	6	NULL	NULL	0	NULL	statement 1	NULL		disrupts	NULL				cell-cell interactions	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_1_303_s_218	10880400	18  In the studies of Lelongt et al, 8  the antibodies and TIMP-1 which bind specifically to gelB may somehow, either directly or indirectly, disrupt cell-cell or cell-matrix interactions that are necessary for branching morphogenesis.	bind
19772	6	6819	6	NULL	NULL	0	NULL	statement 2	NULL		disrupts	NULL				cell-matrix interactions	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_1_303_s_218	10880400	18  In the studies of Lelongt et al, 8  the antibodies and TIMP-1 which bind specifically to gelB may somehow, either directly or indirectly, disrupt cell-cell or cell-matrix interactions that are necessary for branching morphogenesis.	bind
23745	1	6820	5	13	NULL	NULL	NULL	JNK	GP		bind					c-Jun	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_227_s_23	9484987	18  On the other hand, JNK binds to c-Jun to specifically phosphorylate Ser-63 and -73 at the  N-terminal of c-Jun, 19  a major component of AP-1 transcriptional complex.	bind
23746	2	6820	5	13	NULL	NULL	NULL	statement 1	GP		phosphorylates		specifically			c-Jun	GP		Ser-63 at N-terminal		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_227_s_23	9484987	18  On the other hand, JNK binds to c-Jun to specifically phosphorylate Ser-63 and -73 at the  N-terminal of c-Jun, 19  a major component of AP-1 transcriptional complex.	bind
23747	3	6820	5	13	NULL	NULL	NULL	statement 1	GP		phosphorylates		specifically			c-Jun	GP		Ser-73 at N-terminal		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_227_s_23	9484987	18  On the other hand, JNK binds to c-Jun to specifically phosphorylate Ser-63 and -73 at the  N-terminal of c-Jun, 19  a major component of AP-1 transcriptional complex.	bind
23748	4	6820	5	13	NULL	NULL	NULL	statement 1	GP		is a component of		major			AP-1 transcriptional complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_227_s_23	9484987	18  On the other hand, JNK binds to c-Jun to specifically phosphorylate Ser-63 and -73 at the  N-terminal of c-Jun, 19  a major component of AP-1 transcriptional complex.	bind
56605	5	6820	5	13	NULL	NULL	NULL	statement 2	Process		occur simulataneous with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_227_s_23	9484987	18  On the other hand, JNK binds to c-Jun to specifically phosphorylate Ser-63 and -73 at the  N-terminal of c-Jun, 19  a major component of AP-1 transcriptional complex.	bind
19859	1	6820	6	NULL	NULL	0	NULL	JNK	NULL		bind	NULL				c-Jun	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_227_s_23	9484987	18  On the other hand, JNK binds to c-Jun to specifically phosphorylate Ser-63 and -73 at the  N-terminal of c-Jun, 19  a major component of AP-1 transcriptional complex.	bind
19860	2	6820	6	10	NULL	0	NULL	statement 1			phosphorylates		specifically			c-Jun			ser-63 at the N-terminal		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_227_s_23	9484987	18  On the other hand, JNK binds to c-Jun to specifically phosphorylate Ser-63 and -73 at the  N-terminal of c-Jun, 19  a major component of AP-1 transcriptional complex.	bind
19861	3	6820	6	10	NULL	0	NULL	statement 1			phosphorylates		specifically			c-Jun			Ser-73 at the N-terminal		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_227_s_23	9484987	18  On the other hand, JNK binds to c-Jun to specifically phosphorylate Ser-63 and -73 at the  N-terminal of c-Jun, 19  a major component of AP-1 transcriptional complex.	bind
19862	4	6820	6	NULL	NULL	0	NULL	c-Jun	NULL		is a major component of	NULL				AP-1 transcriptional complex	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_227_s_23	9484987	18  On the other hand, JNK binds to c-Jun to specifically phosphorylate Ser-63 and -73 at the  N-terminal of c-Jun, 19  a major component of AP-1 transcriptional complex.	bind
20118	5	6820	6	NULL	NULL	0	NULL	statement 2	NULL		occurs simultaneously with	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_227_s_23	9484987	18  On the other hand, JNK binds to c-Jun to specifically phosphorylate Ser-63 and -73 at the  N-terminal of c-Jun, 19  a major component of AP-1 transcriptional complex.	bind
23749	1	6821	5	13	NULL	NULL	NULL	TAFIa	GP		bind		reduced affinity			plasminogen	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_12_2511_s_93	11116046	18  TAFIa exhibits at least a 10-fold reduced affinity for plasminogen, suggesting that binding to plasminogen is facilitated through the activation peptide, although the physiological role for the interaction has not been elucidated.	bind
23751	2	6821	5	13	NULL	NULL	NULL	statement 1	Process		is facilitated through					activation peptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_12_2511_s_93	11116046	18  TAFIa exhibits at least a 10-fold reduced affinity for plasminogen, suggesting that binding to plasminogen is facilitated through the activation peptide, although the physiological role for the interaction has not been elucidated.	bind
23752	3	6821	5	13	NULL	NULL	NULL	statement 1	Process		suggests					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_12_2511_s_93	11116046	18  TAFIa exhibits at least a 10-fold reduced affinity for plasminogen, suggesting that binding to plasminogen is facilitated through the activation peptide, although the physiological role for the interaction has not been elucidated.	bind
19774	1	6821	6	NULL	NULL	0	NULL	TAFIa	NULL		bind	NULL	reduced affinity			plasminogen	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_12_2511_s_93	11116046	18  TAFIa exhibits at least a 10-fold reduced affinity for plasminogen, suggesting that binding to plasminogen is facilitated through the activation peptide, although the physiological role for the interaction has not been elucidated.	bind
19776	2	6821	6	NULL	NULL	0	NULL	statement 1	NULL		is facilitated through	NULL				activation peptide	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_12_2511_s_93	11116046	18  TAFIa exhibits at least a 10-fold reduced affinity for plasminogen, suggesting that binding to plasminogen is facilitated through the activation peptide, although the physiological role for the interaction has not been elucidated.	bind
56606	3	6821	6	10	NULL	0	NULL	statement 1			suggests					statement 2					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_12_2511_s_93	11116046	18  TAFIa exhibits at least a 10-fold reduced affinity for plasminogen, suggesting that binding to plasminogen is facilitated through the activation peptide, although the physiological role for the interaction has not been elucidated.	bind
23753	1	6822	5	13	NULL	NULL	NULL	myosin	GP		bind		weakly			actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_2_439_s_115	7614728	18  The hydrolysis step is believed to occur while the myosin is weakly bound to actin (ie, when the myosin rapidly attaches and detaches from actin).	bind
23754	2	6822	5	13	NULL	NULL	NULL	statement 1	Process		leads to					hydrolysis	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_2_439_s_115	7614728	18  The hydrolysis step is believed to occur while the myosin is weakly bound to actin (ie, when the myosin rapidly attaches and detaches from actin).	bind
19785	1	6822	6	NULL	NULL	0	NULL	myosin	NULL		bind	NULL	weakly			actin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_77_2_439_s_115	7614728	18  The hydrolysis step is believed to occur while the myosin is weakly bound to actin (ie, when the myosin rapidly attaches and detaches from actin).	bind
19786	2	6822	6	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				hydrolysis	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_77_2_439_s_115	7614728	18  The hydrolysis step is believed to occur while the myosin is weakly bound to actin (ie, when the myosin rapidly attaches and detaches from actin).	bind
23755	1	6823	5	13	NULL	NULL	NULL	apo(a)	GP		bind								lysine		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_575_s_210	10669658	18  The mechanism by which Lp(a) may favor the atherothrombotic process may be related to the lysine-binding properties of apo(a).	bind
23756	2	6823	5	13	NULL	NULL	NULL	Lp(a)	GP		favor		may			atherothrombosis	MedicalFinding	process of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_575_s_210	10669658	18  The mechanism by which Lp(a) may favor the atherothrombotic process may be related to the lysine-binding properties of apo(a).	bind
23757	3	6823	5	13	NULL	NULL	NULL	statement 2	Process	mechanism of	related to		may be			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_575_s_210	10669658	18  The mechanism by which Lp(a) may favor the atherothrombotic process may be related to the lysine-binding properties of apo(a).	bind
19787	1	6823	6	NULL	NULL	0	NULL	apo(a)	NULL		bind	NULL				lysine	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_575_s_210	10669658	18  The mechanism by which Lp(a) may favor the atherothrombotic process may be related to the lysine-binding properties of apo(a).	bind
19788	2	6823	6	10	NULL	0	NULL	Lp(a)			favour					atherothrombosis		process of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_575_s_210	10669658	18  The mechanism by which Lp(a) may favor the atherothrombotic process may be related to the lysine-binding properties of apo(a).	bind
19789	3	6823	6	10	NULL	0	NULL	statement 2			related to		may be			statement 1					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_575_s_210	10669658	18  The mechanism by which Lp(a) may favor the atherothrombotic process may be related to the lysine-binding properties of apo(a).	bind
23758	1	6824	5	13	NULL	NULL	NULL	CsA	Chemical		bind					immunophilin proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_20_2431_s_157	10821822	18  The significant biological effects in common to both CsA and FK506, which each bind different immunophilin proteins, have been attributed to their ability to inhibit calcineurin.	bind
23759	2	6824	5	13	NULL	NULL	NULL	FK506	Chemical		bind					immunophilin proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_20_2431_s_157	10821822	18  The significant biological effects in common to both CsA and FK506, which each bind different immunophilin proteins, have been attributed to their ability to inhibit calcineurin.	bind
23760	3	6824	5	13	NULL	NULL	NULL	CsA	Chemical		inhibit					calcineurin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_20_2431_s_157	10821822	18  The significant biological effects in common to both CsA and FK506, which each bind different immunophilin proteins, have been attributed to their ability to inhibit calcineurin.	bind
23761	4	6824	5	13	NULL	NULL	NULL	FK506	Chemical		inhibit					calcineurin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_20_2431_s_157	10821822	18  The significant biological effects in common to both CsA and FK506, which each bind different immunophilin proteins, have been attributed to their ability to inhibit calcineurin.	bind
23762	5	6824	5	13	NULL	NULL	NULL	statement 1	Process		is attributed to					statement 3	Process	ability of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_20_2431_s_157	10821822	18  The significant biological effects in common to both CsA and FK506, which each bind different immunophilin proteins, have been attributed to their ability to inhibit calcineurin.	bind
23763	6	6824	5	13	NULL	NULL	NULL	statement 2	Process		is attributed to					statement 4	Process	ability of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_20_2431_s_157	10821822	18  The significant biological effects in common to both CsA and FK506, which each bind different immunophilin proteins, have been attributed to their ability to inhibit calcineurin.	bind
19790	1	6824	6	NULL	NULL	0	NULL	CsA	NULL		inhibit	NULL				calcineurin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_101_20_2431_s_157	10821822	18  The significant biological effects in common to both CsA and FK506, which each bind different immunophilin proteins, have been attributed to their ability to inhibit calcineurin.	bind
19791	2	6824	6	NULL	NULL	0	NULL	CsA	NULL		bind	NULL				immunophilin proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_101_20_2431_s_157	10821822	18  The significant biological effects in common to both CsA and FK506, which each bind different immunophilin proteins, have been attributed to their ability to inhibit calcineurin.	bind
19792	3	6824	6	NULL	NULL	0	NULL	FK506	NULL		bind	NULL				immunophilin proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_101_20_2431_s_157	10821822	18  The significant biological effects in common to both CsA and FK506, which each bind different immunophilin proteins, have been attributed to their ability to inhibit calcineurin.	bind
19793	4	6824	6	NULL	NULL	0	NULL	FK506	NULL		inhibit	NULL				calcineurin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_101_20_2431_s_157	10821822	18  The significant biological effects in common to both CsA and FK506, which each bind different immunophilin proteins, have been attributed to their ability to inhibit calcineurin.	bind
56607	5	6824	6	10	NULL	0	NULL	statement 2			is attributed to					statement 1		ability of			NULL		0	NULL	NULL	NULL	gw60_circulation_101_20_2431_s_157	10821822	18  The significant biological effects in common to both CsA and FK506, which each bind different immunophilin proteins, have been attributed to their ability to inhibit calcineurin.	bind
56608	6	6824	6	10	NULL	0	NULL	statement 3			is attributed to					statement 4		ability of			NULL		0	NULL	NULL	NULL	gw60_circulation_101_20_2431_s_157	10821822	18  The significant biological effects in common to both CsA and FK506, which each bind different immunophilin proteins, have been attributed to their ability to inhibit calcineurin.	bind
23764	1	6825	5	13	NULL	NULL	NULL	FGF-1	GP		bind		may			FGFR-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_7_854_s_145	12176960	18 -  21 FGF-1 may bind to 4 FGF receptors, termed FGFR-1, -2, -3, and -4.	bind
23765	2	6825	5	13	NULL	NULL	NULL	FGF-1	GP		bind		may			FGFR-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_7_854_s_145	12176960	18 -  21 FGF-1 may bind to 4 FGF receptors, termed FGFR-1, -2, -3, and -4.	bind
23766	3	6825	5	13	NULL	NULL	NULL	FGF-1	GP		bind		may			FGFR-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_7_854_s_145	12176960	18 -  21 FGF-1 may bind to 4 FGF receptors, termed FGFR-1, -2, -3, and -4.	bind
23767	4	6825	5	13	NULL	NULL	NULL	FGF-1	GP		bind		may			FGFR-4	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_7_854_s_145	12176960	18 -  21 FGF-1 may bind to 4 FGF receptors, termed FGFR-1, -2, -3, and -4.	bind
19794	1	6825	6	NULL	NULL	0	NULL	FGF-1	NULL		bind	NULL	may			FGFR-1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_7_854_s_145	12176960	18 -  21 FGF-1 may bind to 4 FGF receptors, termed FGFR-1, -2, -3, and -4.	bind
19795	2	6825	6	NULL	NULL	0	NULL	FGF-1	NULL		bind	NULL	may			FGFR-2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_7_854_s_145	12176960	18 -  21 FGF-1 may bind to 4 FGF receptors, termed FGFR-1, -2, -3, and -4.	bind
19796	3	6825	6	NULL	NULL	0	NULL	FGF-1	NULL		bind	NULL	may			FGFR-3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_7_854_s_145	12176960	18 -  21 FGF-1 may bind to 4 FGF receptors, termed FGFR-1, -2, -3, and -4.	bind
19797	4	6825	6	NULL	NULL	0	NULL	FGF-1	NULL		bind	NULL	may			FGFR-4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_7_854_s_145	12176960	18 -  21 FGF-1 may bind to 4 FGF receptors, termed FGFR-1, -2, -3, and -4.	bind
23768	1	6826	5	13	NULL	NULL	NULL	LTIP	GP		is					lipid transfer inhibitor protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1716_s_28	9327768	18 - 20 This protein, termed lipid transfer inhibitor protein (LTIP), is characterized as a unique acidic glycoprotein with a molecular weight ranging from 29 000 to 35 000.18,19 Although the mechanism of LTIP is not well understood, binding studies have demonstrated a direct correlation between the suppression of LTP activity by LTIP and the disruption of LTP-lipoprotein binding by this protein,21 suggesting that LTIP inhibits LTP by competing with the transfer protein for the interaction with lipoprotein surface.	bind
23769	2	6826	5	13	NULL	NULL	NULL	LTIP	GP		is characterized as					acidic glycoprotein	GP	unique			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1716_s_28	9327768	18 - 20 This protein, termed lipid transfer inhibitor protein (LTIP), is characterized as a unique acidic glycoprotein with a molecular weight ranging from 29 000 to 35 000.18,19 Although the mechanism of LTIP is not well understood, binding studies have demonstrated a direct correlation between the suppression of LTP activity by LTIP and the disruption of LTP-lipoprotein binding by this protein,21 suggesting that LTIP inhibits LTP by competing with the transfer protein for the interaction with lipoprotein surface.	bind
23770	3	6826	5	13	NULL	NULL	NULL	LTIP	GP		suppresses					LTP	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1716_s_28	9327768	18 - 20 This protein, termed lipid transfer inhibitor protein (LTIP), is characterized as a unique acidic glycoprotein with a molecular weight ranging from 29 000 to 35 000.18,19 Although the mechanism of LTIP is not well understood, binding studies have demonstrated a direct correlation between the suppression of LTP activity by LTIP and the disruption of LTP-lipoprotein binding by this protein,21 suggesting that LTIP inhibits LTP by competing with the transfer protein for the interaction with lipoprotein surface.	bind
23771	4	6826	5	13	NULL	NULL	NULL	LTP	GP		bind					lipoprotein	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1716_s_28	9327768	18 - 20 This protein, termed lipid transfer inhibitor protein (LTIP), is characterized as a unique acidic glycoprotein with a molecular weight ranging from 29 000 to 35 000.18,19 Although the mechanism of LTIP is not well understood, binding studies have demonstrated a direct correlation between the suppression of LTP activity by LTIP and the disruption of LTP-lipoprotein binding by this protein,21 suggesting that LTIP inhibits LTP by competing with the transfer protein for the interaction with lipoprotein surface.	bind
23772	5	6826	5	13	NULL	NULL	NULL	LTIP	GP		disrupt					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1716_s_28	9327768	18 - 20 This protein, termed lipid transfer inhibitor protein (LTIP), is characterized as a unique acidic glycoprotein with a molecular weight ranging from 29 000 to 35 000.18,19 Although the mechanism of LTIP is not well understood, binding studies have demonstrated a direct correlation between the suppression of LTP activity by LTIP and the disruption of LTP-lipoprotein binding by this protein,21 suggesting that LTIP inhibits LTP by competing with the transfer protein for the interaction with lipoprotein surface.	bind
23774	6	6826	5	13	NULL	NULL	NULL	statement 3	Process		correlates with		directly			statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1716_s_28	9327768	18 - 20 This protein, termed lipid transfer inhibitor protein (LTIP), is characterized as a unique acidic glycoprotein with a molecular weight ranging from 29 000 to 35 000.18,19 Although the mechanism of LTIP is not well understood, binding studies have demonstrated a direct correlation between the suppression of LTP activity by LTIP and the disruption of LTP-lipoprotein binding by this protein,21 suggesting that LTIP inhibits LTP by competing with the transfer protein for the interaction with lipoprotein surface.	bind
23775	7	6826	5	13	NULL	NULL	NULL	LTIP	GP		inhibit					LTP	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1716_s_28	9327768	18 - 20 This protein, termed lipid transfer inhibitor protein (LTIP), is characterized as a unique acidic glycoprotein with a molecular weight ranging from 29 000 to 35 000.18,19 Although the mechanism of LTIP is not well understood, binding studies have demonstrated a direct correlation between the suppression of LTP activity by LTIP and the disruption of LTP-lipoprotein binding by this protein,21 suggesting that LTIP inhibits LTP by competing with the transfer protein for the interaction with lipoprotein surface.	bind
23776	8	6826	5	13	NULL	NULL	NULL	LTIP	GP		interacts with					lipoprotein	GP	surface			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1716_s_28	9327768	18 - 20 This protein, termed lipid transfer inhibitor protein (LTIP), is characterized as a unique acidic glycoprotein with a molecular weight ranging from 29 000 to 35 000.18,19 Although the mechanism of LTIP is not well understood, binding studies have demonstrated a direct correlation between the suppression of LTP activity by LTIP and the disruption of LTP-lipoprotein binding by this protein,21 suggesting that LTIP inhibits LTP by competing with the transfer protein for the interaction with lipoprotein surface.	bind
23777	9	6826	5	13	NULL	NULL	NULL	transfer protein	GP		interacts with					lipoprotein	GP	surface			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1716_s_28	9327768	18 - 20 This protein, termed lipid transfer inhibitor protein (LTIP), is characterized as a unique acidic glycoprotein with a molecular weight ranging from 29 000 to 35 000.18,19 Although the mechanism of LTIP is not well understood, binding studies have demonstrated a direct correlation between the suppression of LTP activity by LTIP and the disruption of LTP-lipoprotein binding by this protein,21 suggesting that LTIP inhibits LTP by competing with the transfer protein for the interaction with lipoprotein surface.	bind
23778	10	6826	5	13	NULL	NULL	NULL	statement 8	Process		competes with					statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1716_s_28	9327768	18 - 20 This protein, termed lipid transfer inhibitor protein (LTIP), is characterized as a unique acidic glycoprotein with a molecular weight ranging from 29 000 to 35 000.18,19 Although the mechanism of LTIP is not well understood, binding studies have demonstrated a direct correlation between the suppression of LTP activity by LTIP and the disruption of LTP-lipoprotein binding by this protein,21 suggesting that LTIP inhibits LTP by competing with the transfer protein for the interaction with lipoprotein surface.	bind
23779	11	6826	5	13	NULL	NULL	NULL	statement 6	Process		suggests					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1716_s_28	9327768	18 - 20 This protein, termed lipid transfer inhibitor protein (LTIP), is characterized as a unique acidic glycoprotein with a molecular weight ranging from 29 000 to 35 000.18,19 Although the mechanism of LTIP is not well understood, binding studies have demonstrated a direct correlation between the suppression of LTP activity by LTIP and the disruption of LTP-lipoprotein binding by this protein,21 suggesting that LTIP inhibits LTP by competing with the transfer protein for the interaction with lipoprotein surface.	bind
23780	12	6826	5	13	NULL	NULL	NULL	statement 7	Process		occurs by					statement 10	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1716_s_28	9327768	18 - 20 This protein, termed lipid transfer inhibitor protein (LTIP), is characterized as a unique acidic glycoprotein with a molecular weight ranging from 29 000 to 35 000.18,19 Although the mechanism of LTIP is not well understood, binding studies have demonstrated a direct correlation between the suppression of LTP activity by LTIP and the disruption of LTP-lipoprotein binding by this protein,21 suggesting that LTIP inhibits LTP by competing with the transfer protein for the interaction with lipoprotein surface.	bind
19799	1	6826	6	NULL	NULL	0	NULL	LTIP	NULL		is	NULL				lipid transfer inhibitor protein	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1716_s_28	9327768	18 - 20 This protein, termed lipid transfer inhibitor protein (LTIP), is characterized as a unique acidic glycoprotein with a molecular weight ranging from 29 000 to 35 000.18,19 Although the mechanism of LTIP is not well understood, binding studies have demonstrated a direct correlation between the suppression of LTP activity by LTIP and the disruption of LTP-lipoprotein binding by this protein,21 suggesting that LTIP inhibits LTP by competing with the transfer protein for the interaction with lipoprotein surface.	bind
19800	2	6826	6	NULL	NULL	0	NULL	LTIP	NULL		is characterized as	NULL				acidic glycoprotein	NULL	unique 			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1716_s_28	9327768	18 - 20 This protein, termed lipid transfer inhibitor protein (LTIP), is characterized as a unique acidic glycoprotein with a molecular weight ranging from 29 000 to 35 000.18,19 Although the mechanism of LTIP is not well understood, binding studies have demonstrated a direct correlation between the suppression of LTP activity by LTIP and the disruption of LTP-lipoprotein binding by this protein,21 suggesting that LTIP inhibits LTP by competing with the transfer protein for the interaction with lipoprotein surface.	bind
19801	3	6826	6	NULL	NULL	0	NULL	LTIP	NULL		suppress	NULL				LTP 	NULL	activity of 			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1716_s_28	9327768	18 - 20 This protein, termed lipid transfer inhibitor protein (LTIP), is characterized as a unique acidic glycoprotein with a molecular weight ranging from 29 000 to 35 000.18,19 Although the mechanism of LTIP is not well understood, binding studies have demonstrated a direct correlation between the suppression of LTP activity by LTIP and the disruption of LTP-lipoprotein binding by this protein,21 suggesting that LTIP inhibits LTP by competing with the transfer protein for the interaction with lipoprotein surface.	bind
19802	4	6826	6	NULL	NULL	0	NULL	LTP	NULL		bind	NULL				lipoprotein	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1716_s_28	9327768	18 - 20 This protein, termed lipid transfer inhibitor protein (LTIP), is characterized as a unique acidic glycoprotein with a molecular weight ranging from 29 000 to 35 000.18,19 Although the mechanism of LTIP is not well understood, binding studies have demonstrated a direct correlation between the suppression of LTP activity by LTIP and the disruption of LTP-lipoprotein binding by this protein,21 suggesting that LTIP inhibits LTP by competing with the transfer protein for the interaction with lipoprotein surface.	bind
19806	5	6826	6	NULL	NULL	0	NULL	LTIP	NULL		disrupts	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1716_s_28	9327768	18 - 20 This protein, termed lipid transfer inhibitor protein (LTIP), is characterized as a unique acidic glycoprotein with a molecular weight ranging from 29 000 to 35 000.18,19 Although the mechanism of LTIP is not well understood, binding studies have demonstrated a direct correlation between the suppression of LTP activity by LTIP and the disruption of LTP-lipoprotein binding by this protein,21 suggesting that LTIP inhibits LTP by competing with the transfer protein for the interaction with lipoprotein surface.	bind
19807	6	6826	6	10	NULL	0	NULL	LTIP			inhibit					LTP					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1716_s_28	9327768	18 - 20 This protein, termed lipid transfer inhibitor protein (LTIP), is characterized as a unique acidic glycoprotein with a molecular weight ranging from 29 000 to 35 000.18,19 Although the mechanism of LTIP is not well understood, binding studies have demonstrated a direct correlation between the suppression of LTP activity by LTIP and the disruption of LTP-lipoprotein binding by this protein,21 suggesting that LTIP inhibits LTP by competing with the transfer protein for the interaction with lipoprotein surface.	bind
19808	7	6826	6	10	NULL	0	NULL	statement 3			correlates with		directly			statement 4					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1716_s_28	9327768	18 - 20 This protein, termed lipid transfer inhibitor protein (LTIP), is characterized as a unique acidic glycoprotein with a molecular weight ranging from 29 000 to 35 000.18,19 Although the mechanism of LTIP is not well understood, binding studies have demonstrated a direct correlation between the suppression of LTP activity by LTIP and the disruption of LTP-lipoprotein binding by this protein,21 suggesting that LTIP inhibits LTP by competing with the transfer protein for the interaction with lipoprotein surface.	bind
56609	8	6826	6	10	NULL	0	NULL	LTIP			interacts with					lipoprotein		surface			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1716_s_28	9327768	18 - 20 This protein, termed lipid transfer inhibitor protein (LTIP), is characterized as a unique acidic glycoprotein with a molecular weight ranging from 29 000 to 35 000.18,19 Although the mechanism of LTIP is not well understood, binding studies have demonstrated a direct correlation between the suppression of LTP activity by LTIP and the disruption of LTP-lipoprotein binding by this protein,21 suggesting that LTIP inhibits LTP by competing with the transfer protein for the interaction with lipoprotein surface.	bind
56610	9	6826	6	10	NULL	0	NULL	transfer protein			interacts with					lipoprotein		surface			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1716_s_28	9327768	18 - 20 This protein, termed lipid transfer inhibitor protein (LTIP), is characterized as a unique acidic glycoprotein with a molecular weight ranging from 29 000 to 35 000.18,19 Although the mechanism of LTIP is not well understood, binding studies have demonstrated a direct correlation between the suppression of LTP activity by LTIP and the disruption of LTP-lipoprotein binding by this protein,21 suggesting that LTIP inhibits LTP by competing with the transfer protein for the interaction with lipoprotein surface.	bind
56611	10	6826	6	10	NULL	0	NULL	statement 8			compete with					statement 9					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1716_s_28	9327768	18 - 20 This protein, termed lipid transfer inhibitor protein (LTIP), is characterized as a unique acidic glycoprotein with a molecular weight ranging from 29 000 to 35 000.18,19 Although the mechanism of LTIP is not well understood, binding studies have demonstrated a direct correlation between the suppression of LTP activity by LTIP and the disruption of LTP-lipoprotein binding by this protein,21 suggesting that LTIP inhibits LTP by competing with the transfer protein for the interaction with lipoprotein surface.	bind
56612	11	6826	6	10	NULL	0	NULL	statement 7			suggests					statement 6					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1716_s_28	9327768	18 - 20 This protein, termed lipid transfer inhibitor protein (LTIP), is characterized as a unique acidic glycoprotein with a molecular weight ranging from 29 000 to 35 000.18,19 Although the mechanism of LTIP is not well understood, binding studies have demonstrated a direct correlation between the suppression of LTP activity by LTIP and the disruption of LTP-lipoprotein binding by this protein,21 suggesting that LTIP inhibits LTP by competing with the transfer protein for the interaction with lipoprotein surface.	bind
56613	12	6826	6	10	NULL	0	NULL	statement 6			occur by					statement 10					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1716_s_28	9327768	18 - 20 This protein, termed lipid transfer inhibitor protein (LTIP), is characterized as a unique acidic glycoprotein with a molecular weight ranging from 29 000 to 35 000.18,19 Although the mechanism of LTIP is not well understood, binding studies have demonstrated a direct correlation between the suppression of LTP activity by LTIP and the disruption of LTP-lipoprotein binding by this protein,21 suggesting that LTIP inhibits LTP by competing with the transfer protein for the interaction with lipoprotein surface.	bind
23935	1	6827	5	13	NULL	NULL	NULL	EGFR	GP	activated	recruits					Grb2	GP		SH2 domain		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_743_s_65	16574915	18 Activated EGFR recruits the SH2 domain - containing signaling molecule Grb2 ( Growth factor  receptor -  binding protein  2) that, in turn, mediates the binding of EGFR to the E3 ubiquitin ligase c-Cbl to start the cascade of events leading to internalization and degradation.	bind
23936	2	6827	5	13	NULL	NULL	NULL	Grb2	GP		is					Growth factor receptor - binding protein 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_743_s_65	16574915	18 Activated EGFR recruits the SH2 domain - containing signaling molecule Grb2 ( Growth factor  receptor -  binding protein  2) that, in turn, mediates the binding of EGFR to the E3 ubiquitin ligase c-Cbl to start the cascade of events leading to internalization and degradation.	bind
23937	3	6827	5	13	NULL	NULL	NULL	EGFR	GP		bind					c-Cbl	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_743_s_65	16574915	18 Activated EGFR recruits the SH2 domain - containing signaling molecule Grb2 ( Growth factor  receptor -  binding protein  2) that, in turn, mediates the binding of EGFR to the E3 ubiquitin ligase c-Cbl to start the cascade of events leading to internalization and degradation.	bind
23938	4	6827	5	13	NULL	NULL	NULL	statement 1	Process		mediates					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_743_s_65	16574915	18 Activated EGFR recruits the SH2 domain - containing signaling molecule Grb2 ( Growth factor  receptor -  binding protein  2) that, in turn, mediates the binding of EGFR to the E3 ubiquitin ligase c-Cbl to start the cascade of events leading to internalization and degradation.	bind
23939	5	6827	5	13	NULL	NULL	NULL	statement 3	Process		starts					internalization	Process	cascade of events leading to			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_743_s_65	16574915	18 Activated EGFR recruits the SH2 domain - containing signaling molecule Grb2 ( Growth factor  receptor -  binding protein  2) that, in turn, mediates the binding of EGFR to the E3 ubiquitin ligase c-Cbl to start the cascade of events leading to internalization and degradation.	bind
23940	6	6827	5	13	NULL	NULL	NULL	statement 3	Process		starts					degradation	Process	cascade of events leading to			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_743_s_65	16574915	18 Activated EGFR recruits the SH2 domain - containing signaling molecule Grb2 ( Growth factor  receptor -  binding protein  2) that, in turn, mediates the binding of EGFR to the E3 ubiquitin ligase c-Cbl to start the cascade of events leading to internalization and degradation.	bind
56614	7	6827	5	13	NULL	NULL	NULL	c-Cbl	GP		is a type of					E3 ubiquitin ligase	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_743_s_65	16574915	18 Activated EGFR recruits the SH2 domain - containing signaling molecule Grb2 ( Growth factor  receptor -  binding protein  2) that, in turn, mediates the binding of EGFR to the E3 ubiquitin ligase c-Cbl to start the cascade of events leading to internalization and degradation.	bind
19809	1	6827	6	NULL	NULL	0	NULL	EGFR	NULL	activated	recruits	NULL				Grb2	NULL		SH2 domain		NULL		0	NULL	NULL	NULL	gw70_circulationres_98_6_743_s_65	16574915	18 Activated EGFR recruits the SH2 domain - containing signaling molecule Grb2 ( Growth factor  receptor -  binding protein  2) that, in turn, mediates the binding of EGFR to the E3 ubiquitin ligase c-Cbl to start the cascade of events leading to internalization and degradation.	bind
19810	2	6827	6	NULL	NULL	0	NULL	Grb2	NULL		is	NULL				Growth factor receptor - binding protein 2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_6_743_s_65	16574915	18 Activated EGFR recruits the SH2 domain - containing signaling molecule Grb2 ( Growth factor  receptor -  binding protein  2) that, in turn, mediates the binding of EGFR to the E3 ubiquitin ligase c-Cbl to start the cascade of events leading to internalization and degradation.	bind
19811	3	6827	6	NULL	NULL	0	NULL	EGFR	NULL		bind	NULL				c-Cbl	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_6_743_s_65	16574915	18 Activated EGFR recruits the SH2 domain - containing signaling molecule Grb2 ( Growth factor  receptor -  binding protein  2) that, in turn, mediates the binding of EGFR to the E3 ubiquitin ligase c-Cbl to start the cascade of events leading to internalization and degradation.	bind
19812	4	6827	6	10	NULL	0	NULL	c-Cbl			is a type of					E3 ubiquitin ligase					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_743_s_65	16574915	18 Activated EGFR recruits the SH2 domain - containing signaling molecule Grb2 ( Growth factor  receptor -  binding protein  2) that, in turn, mediates the binding of EGFR to the E3 ubiquitin ligase c-Cbl to start the cascade of events leading to internalization and degradation.	bind
19813	5	6827	6	10	NULL	0	NULL	statement 1			mediates					statement 3					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_743_s_65	16574915	18 Activated EGFR recruits the SH2 domain - containing signaling molecule Grb2 ( Growth factor  receptor -  binding protein  2) that, in turn, mediates the binding of EGFR to the E3 ubiquitin ligase c-Cbl to start the cascade of events leading to internalization and degradation.	bind
56615	6	6827	6	10	NULL	0	NULL	statement 3			starts					internalization		cascade of events leading to			NULL		0	NULL	NULL	NULL	gw70_circulationres_98_6_743_s_65	16574915	18 Activated EGFR recruits the SH2 domain - containing signaling molecule Grb2 ( Growth factor  receptor -  binding protein  2) that, in turn, mediates the binding of EGFR to the E3 ubiquitin ligase c-Cbl to start the cascade of events leading to internalization and degradation.	bind
56616	7	6827	6	10	NULL	0	NULL	statement 3			starts					degradation		cascade of events leading to			NULL		0	NULL	NULL	NULL	gw70_circulationres_98_6_743_s_65	16574915	18 Activated EGFR recruits the SH2 domain - containing signaling molecule Grb2 ( Growth factor  receptor -  binding protein  2) that, in turn, mediates the binding of EGFR to the E3 ubiquitin ligase c-Cbl to start the cascade of events leading to internalization and degradation.	bind
23941	1	6828	5	13	NULL	NULL	NULL	factor Xa	GP		bind					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3320_s_220	10652320	18 and  35), most likely, a similar number of ionic contacts participate in the binding of factor Xa to heparin.	bind
23942	2	6828	5	13	NULL	NULL	NULL	ionic contacts	Process		participate in					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3320_s_220	10652320	18 and  35), most likely, a similar number of ionic contacts participate in the binding of factor Xa to heparin.	bind
19814	1	6828	6	NULL	NULL	0	NULL	factor Xa	NULL		bind	NULL				heparin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_5_3320_s_220	10652320	18 and  35), most likely, a similar number of ionic contacts participate in the binding of factor Xa to heparin.	bind
19815	2	6828	6	NULL	NULL	0	NULL	ionic contacts	NULL		participate in	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_5_3320_s_220	10652320	18 and  35), most likely, a similar number of ionic contacts participate in the binding of factor Xa to heparin.	bind
23943	1	6829	5	13	NULL	NULL	NULL	FasL	GP		bind					Fas	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_1_102_s_176	15499040	18 Binding of FasL to Fas in many cells leads to apoptosis of the Fas-bearing cell through mechanisms involving activation of caspases, particularly caspase-8.	bind
23944	2	6829	5	13	NULL	NULL	NULL	statement 1	Process		leads to					Fas-bearing cell	Cell	apoptosis of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_1_102_s_176	15499040	18 Binding of FasL to Fas in many cells leads to apoptosis of the Fas-bearing cell through mechanisms involving activation of caspases, particularly caspase-8.	bind
23945	3	6829	5	13	NULL	NULL	NULL	statement 2	Process		occurs through					caspases	GP	mechanisms involving activation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_1_102_s_176	15499040	18 Binding of FasL to Fas in many cells leads to apoptosis of the Fas-bearing cell through mechanisms involving activation of caspases, particularly caspase-8.	bind
23946	4	6829	5	13	NULL	NULL	NULL	statement 2	Process		occurs through		particularly			caspase-8	GP	mechanisms involving activation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_1_102_s_176	15499040	18 Binding of FasL to Fas in many cells leads to apoptosis of the Fas-bearing cell through mechanisms involving activation of caspases, particularly caspase-8.	bind
19863	1	6829	6	NULL	NULL	0	NULL	FasL	NULL		bind	NULL				Fas	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_1_102_s_176	15499040	18 Binding of FasL to Fas in many cells leads to apoptosis of the Fas-bearing cell through mechanisms involving activation of caspases, particularly caspase-8.	bind
19864	2	6829	6	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				Fas-bearing cell	NULL	apoptosis of 			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_1_102_s_176	15499040	18 Binding of FasL to Fas in many cells leads to apoptosis of the Fas-bearing cell through mechanisms involving activation of caspases, particularly caspase-8.	bind
19865	3	6829	6	NULL	NULL	0	NULL	statement 2	NULL		occurs via	NULL				caspases	NULL	activation of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_1_102_s_176	15499040	18 Binding of FasL to Fas in many cells leads to apoptosis of the Fas-bearing cell through mechanisms involving activation of caspases, particularly caspase-8.	bind
56617	4	6829	6	10	NULL	0	NULL	statement 2			occur through		particularly			caspase-8		activation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_1_102_s_176	15499040	18 Binding of FasL to Fas in many cells leads to apoptosis of the Fas-bearing cell through mechanisms involving activation of caspases, particularly caspase-8.	bind
23947	1	6830	5	13	NULL	NULL	NULL	srGAP1	GP		bind					Cdc42	GP				NULL	in HEK cells expressing Robo1	NULL	NULL	NULL	NULL	gw70_circulationres_98_4_480_s_231	16439689	18 In HEK cells expressing Robo1, srGAP1 binds to Cdc42 and RhoA. 18 However, srGAPs neither bind to nor regulate Rac1, 18 and therefore they are unlikely to provide a direct link between Robo and Rac1 in VSMCs.	bind
23948	2	6830	5	13	NULL	NULL	NULL	srGAP1	GP		bind					RhoA	GP				NULL	in HEK cells expressing Robo1	NULL	NULL	NULL	NULL	gw70_circulationres_98_4_480_s_231	16439689	18 In HEK cells expressing Robo1, srGAP1 binds to Cdc42 and RhoA. 18 However, srGAPs neither bind to nor regulate Rac1, 18 and therefore they are unlikely to provide a direct link between Robo and Rac1 in VSMCs.	bind
23949	3	6830	5	13	NULL	NULL	NULL	srGAPs	GP		does not bind					Rac1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_4_480_s_231	16439689	18 In HEK cells expressing Robo1, srGAP1 binds to Cdc42 and RhoA. 18 However, srGAPs neither bind to nor regulate Rac1, 18 and therefore they are unlikely to provide a direct link between Robo and Rac1 in VSMCs.	bind
23950	4	6830	5	13	NULL	NULL	NULL	srGAPs	GP		does not regulate					Rac1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_4_480_s_231	16439689	18 In HEK cells expressing Robo1, srGAP1 binds to Cdc42 and RhoA. 18 However, srGAPs neither bind to nor regulate Rac1, 18 and therefore they are unlikely to provide a direct link between Robo and Rac1 in VSMCs.	bind
19866	1	6830	6	NULL	NULL	0	NULL	srGAP1	NULL		bind	NULL				Cdc42	NULL				NULL	statement 3	NULL	NULL	NULL	NULL	gw70_circulationres_98_4_480_s_231	16439689	18 In HEK cells expressing Robo1, srGAP1 binds to Cdc42 and RhoA. 18 However, srGAPs neither bind to nor regulate Rac1, 18 and therefore they are unlikely to provide a direct link between Robo and Rac1 in VSMCs.	bind
19867	2	6830	6	NULL	NULL	0	NULL	srGAP1	NULL		bind	NULL				RhoA	NULL				NULL	statement 3	NULL	NULL	NULL	NULL	gw70_circulationres_98_4_480_s_231	16439689	18 In HEK cells expressing Robo1, srGAP1 binds to Cdc42 and RhoA. 18 However, srGAPs neither bind to nor regulate Rac1, 18 and therefore they are unlikely to provide a direct link between Robo and Rac1 in VSMCs.	bind
19868	3	6830	6	NULL	NULL	0	NULL	HEK cells	NULL		express	NULL				Robo1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_4_480_s_231	16439689	18 In HEK cells expressing Robo1, srGAP1 binds to Cdc42 and RhoA. 18 However, srGAPs neither bind to nor regulate Rac1, 18 and therefore they are unlikely to provide a direct link between Robo and Rac1 in VSMCs.	bind
19869	4	6830	6	NULL	NULL	0	NULL	srGAP	NULL		does not bind	NULL				Rac1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_4_480_s_231	16439689	18 In HEK cells expressing Robo1, srGAP1 binds to Cdc42 and RhoA. 18 However, srGAPs neither bind to nor regulate Rac1, 18 and therefore they are unlikely to provide a direct link between Robo and Rac1 in VSMCs.	bind
19870	5	6830	6	NULL	NULL	0	NULL	srGAP	NULL		does not regulate	NULL				Rac1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_4_480_s_231	16439689	18 In HEK cells expressing Robo1, srGAP1 binds to Cdc42 and RhoA. 18 However, srGAPs neither bind to nor regulate Rac1, 18 and therefore they are unlikely to provide a direct link between Robo and Rac1 in VSMCs.	bind
23952	1	6832	5	13	NULL	NULL	NULL	neuregulins	GP	locally produced	promote					cardiac myocytes	Cell	survival of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_1_93_s_173	11772882	18 Locally produced neuregulins promote survival and growth of cardiac myocytes via ErbB2 and B4 receptors, which also bind heparin-binding epidermal growth factor - like factor.	bind
23953	2	6832	5	13	NULL	NULL	NULL	statement 1	Process		via					ErbB2 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_1_93_s_173	11772882	18 Locally produced neuregulins promote survival and growth of cardiac myocytes via ErbB2 and B4 receptors, which also bind heparin-binding epidermal growth factor - like factor.	bind
23955	3	6832	5	13	NULL	NULL	NULL	statement 1	Process		via					ErbB4 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_1_93_s_173	11772882	18 Locally produced neuregulins promote survival and growth of cardiac myocytes via ErbB2 and B4 receptors, which also bind heparin-binding epidermal growth factor - like factor.	bind
23956	4	6832	5	13	NULL	NULL	NULL	neuregulins	GP	locally produced	promote					cardiac myocytes	Cell	growth of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_1_93_s_173	11772882	18 Locally produced neuregulins promote survival and growth of cardiac myocytes via ErbB2 and B4 receptors, which also bind heparin-binding epidermal growth factor - like factor.	bind
23957	5	6832	5	13	NULL	NULL	NULL	statement 4	Process		via					ErbB2 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_1_93_s_173	11772882	18 Locally produced neuregulins promote survival and growth of cardiac myocytes via ErbB2 and B4 receptors, which also bind heparin-binding epidermal growth factor - like factor.	bind
23959	6	6832	5	13	NULL	NULL	NULL	statement 4	Process		via					ErbB4 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_1_93_s_173	11772882	18 Locally produced neuregulins promote survival and growth of cardiac myocytes via ErbB2 and B4 receptors, which also bind heparin-binding epidermal growth factor - like factor.	bind
23960	7	6832	5	13	NULL	NULL	NULL	neuregulins	GP	locally produced	bind					epidermal growth factor - like factor	GP	heparin-binding			NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_1_93_s_173	11772882	18 Locally produced neuregulins promote survival and growth of cardiac myocytes via ErbB2 and B4 receptors, which also bind heparin-binding epidermal growth factor - like factor.	bind
19871	1	6832	6	NULL	NULL	0	NULL	neuregulins	NULL	locally produced	bind	NULL				heparin-binding epidermal growth factor - like factor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_1_93_s_173	11772882	18 Locally produced neuregulins promote survival and growth of cardiac myocytes via ErbB2 and B4 receptors, which also bind heparin-binding epidermal growth factor - like factor.	bind
19872	2	6832	6	NULL	NULL	0	NULL	neuregulins	NULL		promotes	NULL				cardiac myocytes	NULL	survival of 			NULL		0	NULL	NULL	NULL	gw60_circulation_105_1_93_s_173	11772882	18 Locally produced neuregulins promote survival and growth of cardiac myocytes via ErbB2 and B4 receptors, which also bind heparin-binding epidermal growth factor - like factor.	bind
19873	3	6832	6	NULL	NULL	0	NULL	neuregulins	NULL		promotes	NULL				cardiac myocytes	NULL	growth of 			NULL		0	NULL	NULL	NULL	gw60_circulation_105_1_93_s_173	11772882	18 Locally produced neuregulins promote survival and growth of cardiac myocytes via ErbB2 and B4 receptors, which also bind heparin-binding epidermal growth factor - like factor.	bind
19874	4	6832	6	NULL	NULL	0	NULL	statement 2	NULL		occurs via	NULL				ErbB2 receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_1_93_s_173	11772882	18 Locally produced neuregulins promote survival and growth of cardiac myocytes via ErbB2 and B4 receptors, which also bind heparin-binding epidermal growth factor - like factor.	bind
19875	5	6832	6	NULL	NULL	0	NULL	statement 3	NULL		occurs via	NULL				ErbB4 receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_1_93_s_173	11772882	18 Locally produced neuregulins promote survival and growth of cardiac myocytes via ErbB2 and B4 receptors, which also bind heparin-binding epidermal growth factor - like factor.	bind
56618	6	6832	6	10	NULL	0	NULL	statement 2			via					ErbB4 receptor					NULL		0	NULL	NULL	NULL	gw60_circulation_105_1_93_s_173	11772882	18 Locally produced neuregulins promote survival and growth of cardiac myocytes via ErbB2 and B4 receptors, which also bind heparin-binding epidermal growth factor - like factor.	bind
56619	7	6832	6	10	NULL	0	NULL	statement 3			via					ErbB2 receptor					NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_1_93_s_173	11772882	18 Locally produced neuregulins promote survival and growth of cardiac myocytes via ErbB2 and B4 receptors, which also bind heparin-binding epidermal growth factor - like factor.	bind
23962	1	6833	5	13	NULL	NULL	NULL	TGF-betaR2	GP		bind					ligand	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_5_1633_s_29	11073823	18 TGF-betaR2 binds the ligand and forms a complex with TGF-betaR1 which activates intracellular signaling cascades.	bind
23963	2	6833	5	13	NULL	NULL	NULL	statement 1	GP		forms a complex with					TGF-betaR1	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_5_1633_s_29	11073823	18 TGF-betaR2 binds the ligand and forms a complex with TGF-betaR1 which activates intracellular signaling cascades.	bind
23964	3	6833	5	13	NULL	NULL	NULL	statement 2	Process		activates					intracellular signaling cascades	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_5_1633_s_29	11073823	18 TGF-betaR2 binds the ligand and forms a complex with TGF-betaR1 which activates intracellular signaling cascades.	bind
19876	2	6833	6	10	NULL	0	NULL	statement 1			forms a complex with					TGF-betaR1					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_5_1633_s_29	11073823	18 TGF-betaR2 binds the ligand and forms a complex with TGF-betaR1 which activates intracellular signaling cascades.	bind
19877	3	6833	6	10	NULL	0	NULL	statement 2			activates					intracellular signaling cascades					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_5_1633_s_29	11073823	18 TGF-betaR2 binds the ligand and forms a complex with TGF-betaR1 which activates intracellular signaling cascades.	bind
56620	1	6833	6	10	NULL	0	NULL	TGF-betaR2			bind					ligand					NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_5_1633_s_29	11073823	18 TGF-betaR2 binds the ligand and forms a complex with TGF-betaR1 which activates intracellular signaling cascades.	bind
23965	1	6834	5	13	NULL	NULL	NULL	NorR	GP		bind					norA	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jantimicrobchemoth_54_2_364_s_39	15231765	18 The binding of NorR to the  norA promoter is modified in an  arlS -  strain such that increased  norA expression is observed; however, overexpression of  norR in an  arlS+ background also results in increased  norA expression.	bind
23966	2	6834	5	13	NULL	NULL	NULL	NorR	GP	overexpression of	results in					norA	GP	increased expression of			NULL	in an arlS+ background	NULL	NULL	NULL	NULL	gw70_jantimicrobchemoth_54_2_364_s_39	15231765	18 The binding of NorR to the  norA promoter is modified in an  arlS -  strain such that increased  norA expression is observed; however, overexpression of  norR in an  arlS+ background also results in increased  norA expression.	bind
56621	3	6834	5	13	NULL	NULL	NULL	statement 1	Process		increases					norA	GP	expression of			NULL	arlS - strain	NULL	NULL	NULL	NULL	gw70_jantimicrobchemoth_54_2_364_s_39	15231765	18 The binding of NorR to the  norA promoter is modified in an  arlS -  strain such that increased  norA expression is observed; however, overexpression of  norR in an  arlS+ background also results in increased  norA expression.	bind
19878	1	6834	6	NULL	NULL	0	NULL	NorR	NULL		bind	NULL				norA	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_jantimicrobchemoth_54_2_364_s_39	15231765	18 The binding of NorR to the  norA promoter is modified in an  arlS -  strain such that increased  norA expression is observed; however, overexpression of  norR in an  arlS+ background also results in increased  norA expression.	bind
19879	2	6834	6	NULL	NULL	0	NULL	statement 1	NULL		increases	NULL				norA	NULL	expression of 			NULL	arlS - strain 	0	NULL	NULL	NULL	gw70_jantimicrobchemoth_54_2_364_s_39	15231765	18 The binding of NorR to the  norA promoter is modified in an  arlS -  strain such that increased  norA expression is observed; however, overexpression of  norR in an  arlS+ background also results in increased  norA expression.	bind
19880	3	6834	6	10	NULL	0	NULL	norR		overexpression of	results in					norA expression		increased expression of			NULL	arlS+ background	NULL	NULL	NULL	NULL	gw70_jantimicrobchemoth_54_2_364_s_39	15231765	18 The binding of NorR to the  norA promoter is modified in an  arlS -  strain such that increased  norA expression is observed; however, overexpression of  norR in an  arlS+ background also results in increased  norA expression.	bind
23967	1	6835	5	13	NULL	NULL	NULL	VEGF	GP		bind					VEGFR2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_6_692_s_194	12609969	18 The binding of VEGF to VEGFR2 elicits activation of signaling cascades that trigger the biological effects of VEGF.	bind
23968	2	6835	5	13	NULL	NULL	NULL	statement 1	Process		elicits					signaling cascades	Process	activation of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_6_692_s_194	12609969	18 The binding of VEGF to VEGFR2 elicits activation of signaling cascades that trigger the biological effects of VEGF.	bind
23969	3	6835	5	13	NULL	NULL	NULL	statement 2	Process		triggers					VEGF	GP	biological effects of 			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_6_692_s_194	12609969	18 The binding of VEGF to VEGFR2 elicits activation of signaling cascades that trigger the biological effects of VEGF.	bind
19881	1	6835	6	NULL	NULL	0	NULL	VEGF	NULL		bind	NULL				VEGFR2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_92_6_692_s_194	12609969	18 The binding of VEGF to VEGFR2 elicits activation of signaling cascades that trigger the biological effects of VEGF.	bind
19882	2	6835	6	NULL	NULL	0	NULL	statement 1	NULL		elicits	NULL				signaling cascades	NULL	activation of 			NULL		0	NULL	NULL	NULL	gw60_circulationres_92_6_692_s_194	12609969	18 The binding of VEGF to VEGFR2 elicits activation of signaling cascades that trigger the biological effects of VEGF.	bind
19883	3	6835	6	NULL	NULL	0	NULL	statement 2	NULL		trigger	NULL				VEGF	NULL	biological effects of 			NULL		0	NULL	NULL	NULL	gw60_circulationres_92_6_692_s_194	12609969	18 The binding of VEGF to VEGFR2 elicits activation of signaling cascades that trigger the biological effects of VEGF.	bind
23970	1	6836	5	13	NULL	NULL	NULL	EGF-R	GP		bind		initially			caveolin	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1223_s_137	15142861	18 We also reported that EGF-R initially binds caveolin, but this association is disrupted by Ang II stimulation, which is an essential step in transactivation of EGF-R in VSMCs. 3 Thus, Ang II - stimulated recruitment of Rac1 into caveolae/lipid rafts and association with caveolin may be required for activation of Nox-based NAD(P)H oxidase and downstream ROS-dependent signaling events such as EGF-R transactivation.	bind
23971	2	6836	5	13	NULL	NULL	NULL	Ang II	GP	stimulation	disrupt					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1223_s_137	15142861	18 We also reported that EGF-R initially binds caveolin, but this association is disrupted by Ang II stimulation, which is an essential step in transactivation of EGF-R in VSMCs. 3 Thus, Ang II - stimulated recruitment of Rac1 into caveolae/lipid rafts and association with caveolin may be required for activation of Nox-based NAD(P)H oxidase and downstream ROS-dependent signaling events such as EGF-R transactivation.	bind
23972	3	6836	5	13	NULL	NULL	NULL	statement 2	Process		is an essential step in					EGF-R	GP	transactivation of			NULL	in VSMCs	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1223_s_137	15142861	18 We also reported that EGF-R initially binds caveolin, but this association is disrupted by Ang II stimulation, which is an essential step in transactivation of EGF-R in VSMCs. 3 Thus, Ang II - stimulated recruitment of Rac1 into caveolae/lipid rafts and association with caveolin may be required for activation of Nox-based NAD(P)H oxidase and downstream ROS-dependent signaling events such as EGF-R transactivation.	bind
23973	4	6836	5	13	NULL	NULL	NULL	Rac1	GP		is recruited into					caveolae/lipid rafts	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1223_s_137	15142861	18 We also reported that EGF-R initially binds caveolin, but this association is disrupted by Ang II stimulation, which is an essential step in transactivation of EGF-R in VSMCs. 3 Thus, Ang II - stimulated recruitment of Rac1 into caveolae/lipid rafts and association with caveolin may be required for activation of Nox-based NAD(P)H oxidase and downstream ROS-dependent signaling events such as EGF-R transactivation.	bind
23974	5	6836	5	13	NULL	NULL	NULL	Ang II	GP		stimulates					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1223_s_137	15142861	18 We also reported that EGF-R initially binds caveolin, but this association is disrupted by Ang II stimulation, which is an essential step in transactivation of EGF-R in VSMCs. 3 Thus, Ang II - stimulated recruitment of Rac1 into caveolae/lipid rafts and association with caveolin may be required for activation of Nox-based NAD(P)H oxidase and downstream ROS-dependent signaling events such as EGF-R transactivation.	bind
23975	6	6836	5	13	NULL	NULL	NULL	Rac1	GP		associates with					caveolin	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1223_s_137	15142861	18 We also reported that EGF-R initially binds caveolin, but this association is disrupted by Ang II stimulation, which is an essential step in transactivation of EGF-R in VSMCs. 3 Thus, Ang II - stimulated recruitment of Rac1 into caveolae/lipid rafts and association with caveolin may be required for activation of Nox-based NAD(P)H oxidase and downstream ROS-dependent signaling events such as EGF-R transactivation.	bind
23976	7	6836	5	13	NULL	NULL	NULL	Ang II	GP		stimulates					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1223_s_137	15142861	18 We also reported that EGF-R initially binds caveolin, but this association is disrupted by Ang II stimulation, which is an essential step in transactivation of EGF-R in VSMCs. 3 Thus, Ang II - stimulated recruitment of Rac1 into caveolae/lipid rafts and association with caveolin may be required for activation of Nox-based NAD(P)H oxidase and downstream ROS-dependent signaling events such as EGF-R transactivation.	bind
23977	8	6836	5	13	NULL	NULL	NULL	statement 5	Process		is required for		may be			NAD(P)H oxidase	GP	activation of Nox-based			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1223_s_137	15142861	18 We also reported that EGF-R initially binds caveolin, but this association is disrupted by Ang II stimulation, which is an essential step in transactivation of EGF-R in VSMCs. 3 Thus, Ang II - stimulated recruitment of Rac1 into caveolae/lipid rafts and association with caveolin may be required for activation of Nox-based NAD(P)H oxidase and downstream ROS-dependent signaling events such as EGF-R transactivation.	bind
23978	9	6836	5	13	NULL	NULL	NULL	statement 7	Process		is required for		may be			NAD(P)H oxidase	GP	activation of Nox-based			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1223_s_137	15142861	18 We also reported that EGF-R initially binds caveolin, but this association is disrupted by Ang II stimulation, which is an essential step in transactivation of EGF-R in VSMCs. 3 Thus, Ang II - stimulated recruitment of Rac1 into caveolae/lipid rafts and association with caveolin may be required for activation of Nox-based NAD(P)H oxidase and downstream ROS-dependent signaling events such as EGF-R transactivation.	bind
23979	10	6836	5	13	NULL	NULL	NULL	statement 5	Process		is required for		may be			signaling events	Process	downstream ROS-dependent			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1223_s_137	15142861	18 We also reported that EGF-R initially binds caveolin, but this association is disrupted by Ang II stimulation, which is an essential step in transactivation of EGF-R in VSMCs. 3 Thus, Ang II - stimulated recruitment of Rac1 into caveolae/lipid rafts and association with caveolin may be required for activation of Nox-based NAD(P)H oxidase and downstream ROS-dependent signaling events such as EGF-R transactivation.	bind
23980	11	6836	5	13	NULL	NULL	NULL	statement 7	Process		is required for		may be			signaling events	Process	downstream ROS-dependent			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1223_s_137	15142861	18 We also reported that EGF-R initially binds caveolin, but this association is disrupted by Ang II stimulation, which is an essential step in transactivation of EGF-R in VSMCs. 3 Thus, Ang II - stimulated recruitment of Rac1 into caveolae/lipid rafts and association with caveolin may be required for activation of Nox-based NAD(P)H oxidase and downstream ROS-dependent signaling events such as EGF-R transactivation.	bind
23981	12	6836	5	13	NULL	NULL	NULL	signaling events	Process	downstream ROS-dependent 	includes					EGF-R	GP	transactivation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1223_s_137	15142861	18 We also reported that EGF-R initially binds caveolin, but this association is disrupted by Ang II stimulation, which is an essential step in transactivation of EGF-R in VSMCs. 3 Thus, Ang II - stimulated recruitment of Rac1 into caveolae/lipid rafts and association with caveolin may be required for activation of Nox-based NAD(P)H oxidase and downstream ROS-dependent signaling events such as EGF-R transactivation.	bind
19884	1	6836	6	NULL	NULL	0	NULL	EGF-R	NULL		bind	NULL				caveolin	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1223_s_137	15142861	18 We also reported that EGF-R initially binds caveolin, but this association is disrupted by Ang II stimulation, which is an essential step in transactivation of EGF-R in VSMCs. 3 Thus, Ang II - stimulated recruitment of Rac1 into caveolae/lipid rafts and association with caveolin may be required for activation of Nox-based NAD(P)H oxidase and downstream ROS-dependent signaling events such as EGF-R transactivation.	bind
19885	2	6836	6	NULL	NULL	0	NULL	statement 1	NULL		is disrupted by	NULL				Ang II	NULL	stimulation of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1223_s_137	15142861	18 We also reported that EGF-R initially binds caveolin, but this association is disrupted by Ang II stimulation, which is an essential step in transactivation of EGF-R in VSMCs. 3 Thus, Ang II - stimulated recruitment of Rac1 into caveolae/lipid rafts and association with caveolin may be required for activation of Nox-based NAD(P)H oxidase and downstream ROS-dependent signaling events such as EGF-R transactivation.	bind
19886	3	6836	6	NULL	NULL	0	NULL	statement 1	NULL		is essential step for	NULL				EGF-R	NULL	transactivation of			NULL	VSMC	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1223_s_137	15142861	18 We also reported that EGF-R initially binds caveolin, but this association is disrupted by Ang II stimulation, which is an essential step in transactivation of EGF-R in VSMCs. 3 Thus, Ang II - stimulated recruitment of Rac1 into caveolae/lipid rafts and association with caveolin may be required for activation of Nox-based NAD(P)H oxidase and downstream ROS-dependent signaling events such as EGF-R transactivation.	bind
19887	4	6836	6	NULL	NULL	0	NULL	Rac1	NULL		is recruited into	NULL				caveolae/lipid rafts	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1223_s_137	15142861	18 We also reported that EGF-R initially binds caveolin, but this association is disrupted by Ang II stimulation, which is an essential step in transactivation of EGF-R in VSMCs. 3 Thus, Ang II - stimulated recruitment of Rac1 into caveolae/lipid rafts and association with caveolin may be required for activation of Nox-based NAD(P)H oxidase and downstream ROS-dependent signaling events such as EGF-R transactivation.	bind
19888	5	6836	6	NULL	NULL	0	NULL	statement 4	NULL		is stimulated by	NULL				Ang II	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1223_s_137	15142861	18 We also reported that EGF-R initially binds caveolin, but this association is disrupted by Ang II stimulation, which is an essential step in transactivation of EGF-R in VSMCs. 3 Thus, Ang II - stimulated recruitment of Rac1 into caveolae/lipid rafts and association with caveolin may be required for activation of Nox-based NAD(P)H oxidase and downstream ROS-dependent signaling events such as EGF-R transactivation.	bind
19889	6	6836	6	NULL	NULL	0	NULL	Rac1	NULL		associates	NULL				caveolin	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1223_s_137	15142861	18 We also reported that EGF-R initially binds caveolin, but this association is disrupted by Ang II stimulation, which is an essential step in transactivation of EGF-R in VSMCs. 3 Thus, Ang II - stimulated recruitment of Rac1 into caveolae/lipid rafts and association with caveolin may be required for activation of Nox-based NAD(P)H oxidase and downstream ROS-dependent signaling events such as EGF-R transactivation.	bind
19890	7	6836	6	10	NULL	0	NULL	statement 5			be required for		may			 NAD(P)H oxidase		activation of Nox-based			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1223_s_137	15142861	18 We also reported that EGF-R initially binds caveolin, but this association is disrupted by Ang II stimulation, which is an essential step in transactivation of EGF-R in VSMCs. 3 Thus, Ang II - stimulated recruitment of Rac1 into caveolae/lipid rafts and association with caveolin may be required for activation of Nox-based NAD(P)H oxidase and downstream ROS-dependent signaling events such as EGF-R transactivation.	bind
19891	8	6836	6	10	NULL	0	NULL	statement 5			be required for		may			signaling events		downstream ROS-dependent			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1223_s_137	15142861	18 We also reported that EGF-R initially binds caveolin, but this association is disrupted by Ang II stimulation, which is an essential step in transactivation of EGF-R in VSMCs. 3 Thus, Ang II - stimulated recruitment of Rac1 into caveolae/lipid rafts and association with caveolin may be required for activation of Nox-based NAD(P)H oxidase and downstream ROS-dependent signaling events such as EGF-R transactivation.	bind
56622	9	6836	6	10	NULL	0	NULL	Ang II			stimulates					statement 6					NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1223_s_137	15142861	18 We also reported that EGF-R initially binds caveolin, but this association is disrupted by Ang II stimulation, which is an essential step in transactivation of EGF-R in VSMCs. 3 Thus, Ang II - stimulated recruitment of Rac1 into caveolae/lipid rafts and association with caveolin may be required for activation of Nox-based NAD(P)H oxidase and downstream ROS-dependent signaling events such as EGF-R transactivation.	bind
56623	10	6836	6	10	NULL	0	NULL	statement 9			be required for		may			NAD(P)H oxidase		activation of Nox-based			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1223_s_137	15142861	18 We also reported that EGF-R initially binds caveolin, but this association is disrupted by Ang II stimulation, which is an essential step in transactivation of EGF-R in VSMCs. 3 Thus, Ang II - stimulated recruitment of Rac1 into caveolae/lipid rafts and association with caveolin may be required for activation of Nox-based NAD(P)H oxidase and downstream ROS-dependent signaling events such as EGF-R transactivation.	bind
56624	11	6836	6	10	NULL	0	NULL	statement 9			be required for		may			signaling events		downstream ROS-dependent 			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1223_s_137	15142861	18 We also reported that EGF-R initially binds caveolin, but this association is disrupted by Ang II stimulation, which is an essential step in transactivation of EGF-R in VSMCs. 3 Thus, Ang II - stimulated recruitment of Rac1 into caveolae/lipid rafts and association with caveolin may be required for activation of Nox-based NAD(P)H oxidase and downstream ROS-dependent signaling events such as EGF-R transactivation.	bind
56625	12	6836	6	10	NULL	0	NULL	signaling events		ROS-dependent 	include					EGF-R		transactivation of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1223_s_137	15142861	18 We also reported that EGF-R initially binds caveolin, but this association is disrupted by Ang II stimulation, which is an essential step in transactivation of EGF-R in VSMCs. 3 Thus, Ang II - stimulated recruitment of Rac1 into caveolae/lipid rafts and association with caveolin may be required for activation of Nox-based NAD(P)H oxidase and downstream ROS-dependent signaling events such as EGF-R transactivation.	bind
23982	1	6837	5	13	NULL	NULL	NULL	CD36 	GP	expression of	function as					TSP-1 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_3_841_s_315	10487979	18, 19  No previous report has demonstrated that CD36 binds TGF-beta1, but CD36 expression functions as a receptor for TSP-1, 43  collagen, 43  and a ligand exposed on the surface of erythrocytes infected with the parasite  Plasmodium falciparum.	bind
23983	2	6837	5	13	NULL	NULL	NULL	CD36	GP	expression of	function as					collagen receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_3_841_s_315	10487979	18, 19  No previous report has demonstrated that CD36 binds TGF-beta1, but CD36 expression functions as a receptor for TSP-1, 43  collagen, 43  and a ligand exposed on the surface of erythrocytes infected with the parasite  Plasmodium falciparum.	bind
23984	3	6837	5	13	NULL	NULL	NULL	CD36	GP	expression of	function as					ligand receptor	GP				NULL	surface of erythrocytes infected with the parasite Plasmodium falciparum	NULL	NULL	NULL	NULL	gw60_amjpathol_155_3_841_s_315	10487979	18, 19  No previous report has demonstrated that CD36 binds TGF-beta1, but CD36 expression functions as a receptor for TSP-1, 43  collagen, 43  and a ligand exposed on the surface of erythrocytes infected with the parasite  Plasmodium falciparum.	bind
19892	1	6837	6	NULL	NULL	0	NULL	CD36	NULL	expression of	functions as 	NULL				TSP-1 receptor	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_3_841_s_315	10487979	18, 19  No previous report has demonstrated that CD36 binds TGF-beta1, but CD36 expression functions as a receptor for TSP-1, 43  collagen, 43  and a ligand exposed on the surface of erythrocytes infected with the parasite  Plasmodium falciparum.	bind
20292	2	6837	6	NULL	NULL	0	NULL	CD36	NULL	expression of	functions as 	NULL				collagen receptor	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_3_841_s_315	10487979	18, 19  No previous report has demonstrated that CD36 binds TGF-beta1, but CD36 expression functions as a receptor for TSP-1, 43  collagen, 43  and a ligand exposed on the surface of erythrocytes infected with the parasite  Plasmodium falciparum.	bind
20294	3	6837	6	NULL	NULL	0	NULL	CD36	NULL	expression of	functions as a 	NULL				ligand receptor	NULL				NULL	surface of erythrocytes infected with the parasite Plasmodium falciparum	NULL	NULL	NULL	NULL	gw60_amjpathol_155_3_841_s_315	10487979	18, 19  No previous report has demonstrated that CD36 binds TGF-beta1, but CD36 expression functions as a receptor for TSP-1, 43  collagen, 43  and a ligand exposed on the surface of erythrocytes infected with the parasite  Plasmodium falciparum.	bind
23986	1	6838	5	13	NULL	NULL	NULL	VEGF	GP		bind					Flt-1	GP				NULL	vascular endothelial cells	NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_103_s_21	10880381	18, 19  VEGF binds to two type III tyrosine kinase receptors on vascular endothelial cells, Flt-1 and KDR/Flk-1.	bind
23987	2	6838	5	13	NULL	NULL	NULL	VEGF	GP		bind					KDR/Flk-1	GP				NULL	vascular endothelial cells	NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_103_s_21	10880381	18, 19  VEGF binds to two type III tyrosine kinase receptors on vascular endothelial cells, Flt-1 and KDR/Flk-1.	bind
30346	3	6838	5	13	NULL	NULL	NULL	Flt-1	GP		is a type of					type III tyrosine kinase receptors 	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_103_s_21	10880381	18, 19  VEGF binds to two type III tyrosine kinase receptors on vascular endothelial cells, Flt-1 and KDR/Flk-1.	bind
30347	4	6838	5	13	NULL	NULL	NULL	KDR/Flk-1	GP		is a type of					type III tyrosine kinase receptors 	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_103_s_21	10880381	18, 19  VEGF binds to two type III tyrosine kinase receptors on vascular endothelial cells, Flt-1 and KDR/Flk-1.	bind
19893	1	6838	6	NULL	NULL	0	NULL	VEGF	NULL		bind	NULL				Flt-1	NULL				NULL	vascular endothelial cells	NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_103_s_21	10880381	18, 19  VEGF binds to two type III tyrosine kinase receptors on vascular endothelial cells, Flt-1 and KDR/Flk-1.	bind
19894	2	6838	6	NULL	NULL	0	NULL	VEGF	NULL		bind	NULL				KDR/Flk-1	NULL				NULL	vascular endothelial cells	0	NULL	NULL	NULL	gw60_amjpathol_157_1_103_s_21	10880381	18, 19  VEGF binds to two type III tyrosine kinase receptors on vascular endothelial cells, Flt-1 and KDR/Flk-1.	bind
19895	3	6838	6	NULL	NULL	0	NULL	Flt-1	NULL		is a type of	NULL				type III tyrosine kinase receptors	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_103_s_21	10880381	18, 19  VEGF binds to two type III tyrosine kinase receptors on vascular endothelial cells, Flt-1 and KDR/Flk-1.	bind
19897	4	6838	6	NULL	NULL	0	NULL	KDR/Flk-1	NULL		is a type of	NULL				type III tyrosine kinase receptors	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_103_s_21	10880381	18, 19  VEGF binds to two type III tyrosine kinase receptors on vascular endothelial cells, Flt-1 and KDR/Flk-1.	bind
23988	1	6839	5	13	NULL	NULL	NULL	CD36	GP		bind					TSP-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_3_841_s_151	10487979	18, 19  We next determined if the CD36 binding of TSP-1 is required for the posttranslational processing and activation of L-TGF- beta1.	bind
19898	1	6839	6	NULL	NULL	0	NULL	CD36	NULL		bind	NULL				TSP-1	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_3_841_s_151	10487979	18, 19  We next determined if the CD36 binding of TSP-1 is required for the posttranslational processing and activation of L-TGF- beta1.	bind
23992	4	6840	5	13	NULL	NULL	NULL	statement 3	Process		enhances					actin filaments	GP	polymerization of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_12_1296_s_25	12775580	18,19  By inducing cofilin phosphorylation, Rho abolishes the actin-binding activity of cofilin, thereby enhancing the polymerization of actin filaments.	bind
30348	1	6840	5	13	NULL	NULL	NULL	Rho	GP		induces					cofilin	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_12_1296_s_25	12775580	18,19  By inducing cofilin phosphorylation, Rho abolishes the actin-binding activity of cofilin, thereby enhancing the polymerization of actin filaments.	bind
30349	2	6840	5	13	NULL	NULL	NULL	cofilin	GP		activates					actin-binding	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_12_1296_s_25	12775580	18,19  By inducing cofilin phosphorylation, Rho abolishes the actin-binding activity of cofilin, thereby enhancing the polymerization of actin filaments.	bind
30350	3	6840	5	13	NULL	NULL	NULL	statement 1	Process		abolishes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_12_1296_s_25	12775580	18,19  By inducing cofilin phosphorylation, Rho abolishes the actin-binding activity of cofilin, thereby enhancing the polymerization of actin filaments.	bind
19899	1	6840	6	NULL	NULL	0	NULL	Rho	NULL		induces	NULL				cofilin	NULL	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_circulationres_92_12_1296_s_25	12775580	18,19  By inducing cofilin phosphorylation, Rho abolishes the actin-binding activity of cofilin, thereby enhancing the polymerization of actin filaments.	bind
19900	2	6840	6	10	NULL	0	NULL	Cofilin			activates					actin-binding					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_12_1296_s_25	12775580	18,19  By inducing cofilin phosphorylation, Rho abolishes the actin-binding activity of cofilin, thereby enhancing the polymerization of actin filaments.	bind
19901	3	6840	6	NULL	NULL	0	NULL	statement 1	NULL		abolishes	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_92_12_1296_s_25	12775580	18,19  By inducing cofilin phosphorylation, Rho abolishes the actin-binding activity of cofilin, thereby enhancing the polymerization of actin filaments.	bind
19902	4	6840	6	NULL	NULL	0	NULL	statement 3	NULL		enhances	NULL				actin filaments	NULL	polymerization of 			NULL		0	NULL	NULL	NULL	gw60_circulationres_92_12_1296_s_25	12775580	18,19  By inducing cofilin phosphorylation, Rho abolishes the actin-binding activity of cofilin, thereby enhancing the polymerization of actin filaments.	bind
23993	1	6842	5	13	NULL	NULL	NULL	PKCalpha	GP		bind					syndecan-4	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_7_674_s_31	16141413	18,19 alpha-Actinin may compete with PKCalpha for binding to syndecan-4 because the increased association of phorbol 12-myristate 13-acetate - activated PKCalpha with syndecan-4 is accompanied by decreased alpha-actinin binding to syndecan-4.	bind
23994	2	6842	5	13	NULL	NULL	NULL	alpha-Actinin	GP		bind					syndecan-4	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_7_674_s_31	16141413	18,19 alpha-Actinin may compete with PKCalpha for binding to syndecan-4 because the increased association of phorbol 12-myristate 13-acetate - activated PKCalpha with syndecan-4 is accompanied by decreased alpha-actinin binding to syndecan-4.	bind
23995	3	6842	5	13	NULL	NULL	NULL	statement 2	Process		competes with		may			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_7_674_s_31	16141413	18,19 alpha-Actinin may compete with PKCalpha for binding to syndecan-4 because the increased association of phorbol 12-myristate 13-acetate - activated PKCalpha with syndecan-4 is accompanied by decreased alpha-actinin binding to syndecan-4.	bind
23996	4	6842	5	13	NULL	NULL	NULL	phorbol 12-myristate 13-acetate	Chemical		activates					PKCalpha	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_7_674_s_31	16141413	18,19 alpha-Actinin may compete with PKCalpha for binding to syndecan-4 because the increased association of phorbol 12-myristate 13-acetate - activated PKCalpha with syndecan-4 is accompanied by decreased alpha-actinin binding to syndecan-4.	bind
23997	5	6842	5	13	NULL	NULL	NULL	statement 4	Process		associates with					syndecan-4	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_7_674_s_31	16141413	18,19 alpha-Actinin may compete with PKCalpha for binding to syndecan-4 because the increased association of phorbol 12-myristate 13-acetate - activated PKCalpha with syndecan-4 is accompanied by decreased alpha-actinin binding to syndecan-4.	bind
23998	6	6842	5	13	NULL	NULL	NULL	statement 5	Process	increased	is accompanied by					statement 2	Process	decreased			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_7_674_s_31	16141413	18,19 alpha-Actinin may compete with PKCalpha for binding to syndecan-4 because the increased association of phorbol 12-myristate 13-acetate - activated PKCalpha with syndecan-4 is accompanied by decreased alpha-actinin binding to syndecan-4.	bind
19903	1	6842	6	NULL	NULL	0	NULL	PKCalpha	NULL		bind	NULL				syndecan-4	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_7_674_s_31	16141413	18,19 alpha-Actinin may compete with PKCalpha for binding to syndecan-4 because the increased association of phorbol 12-myristate 13-acetate - activated PKCalpha with syndecan-4 is accompanied by decreased alpha-actinin binding to syndecan-4.	bind
19904	2	6842	6	NULL	NULL	0	NULL	alpha-Actinin	NULL		bind	NULL				syndecan-4	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_7_674_s_31	16141413	18,19 alpha-Actinin may compete with PKCalpha for binding to syndecan-4 because the increased association of phorbol 12-myristate 13-acetate - activated PKCalpha with syndecan-4 is accompanied by decreased alpha-actinin binding to syndecan-4.	bind
19905	3	6842	6	NULL	NULL	0	NULL	statement 1	NULL		competes	NULL	may			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_7_674_s_31	16141413	18,19 alpha-Actinin may compete with PKCalpha for binding to syndecan-4 because the increased association of phorbol 12-myristate 13-acetate - activated PKCalpha with syndecan-4 is accompanied by decreased alpha-actinin binding to syndecan-4.	bind
19906	4	6842	6	10	NULL	0	NULL	PKCalpha		activated	associate with					syndecan-4					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_7_674_s_31	16141413	18,19 alpha-Actinin may compete with PKCalpha for binding to syndecan-4 because the increased association of phorbol 12-myristate 13-acetate - activated PKCalpha with syndecan-4 is accompanied by decreased alpha-actinin binding to syndecan-4.	bind
19907	5	6842	6	NULL	NULL	0	NULL	statement 4	NULL	increase in	leads to	NULL				statement 2	NULL	decrease in			NULL		0	NULL	NULL	NULL	gw70_circulationres_97_7_674_s_31	16141413	18,19 alpha-Actinin may compete with PKCalpha for binding to syndecan-4 because the increased association of phorbol 12-myristate 13-acetate - activated PKCalpha with syndecan-4 is accompanied by decreased alpha-actinin binding to syndecan-4.	bind
30287	6	6842	6	NULL	NULL	0	NULL	phorbol 12-myristate 13-acetate	NULL		activates	NULL				PKCalpha	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_7_674_s_31	16141413	18,19 alpha-Actinin may compete with PKCalpha for binding to syndecan-4 because the increased association of phorbol 12-myristate 13-acetate - activated PKCalpha with syndecan-4 is accompanied by decreased alpha-actinin binding to syndecan-4.	bind
23999	1	6843	5	13	NULL	NULL	NULL	HDL	GP		bind					SR-BI	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_5_712_s_91	12615688	18,31  There is a half-maximal efflux at low concentrations of HDL (<30 mug protein/mL) that is similar to the Kd for HDL binding to SR-BI.	bind
19908	1	6843	6	NULL	NULL	0	NULL	HDL	NULL		bind	NULL				SR-BI	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_5_712_s_91	12615688	18,31  There is a half-maximal efflux at low concentrations of HDL (<30 mug protein/mL) that is similar to the Kd for HDL binding to SR-BI.	bind
24001	1	6844	5	13	NULL	NULL	NULL	I-LPL	GP		bind					LDL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_14_8081_s_154	7713910	181 nM  unlabeled LDL inhibited  the binding of  I-LPL to LDL-coated plates by  approximately 50%  in both control and delipidated plates.	bind
24002	2	6844	5	13	NULL	NULL	NULL	LDL	GP	unlabeled	inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_14_8081_s_154	7713910	181 nM  unlabeled LDL inhibited  the binding of  I-LPL to LDL-coated plates by  approximately 50%  in both control and delipidated plates.	bind
19909	1	6844	6	NULL	NULL	0	NULL	I-LPL	NULL		bind	NULL				LDL	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_14_8081_s_154	7713910	181 nM  unlabeled LDL inhibited  the binding of  I-LPL to LDL-coated plates by  approximately 50%  in both control and delipidated plates.	bind
19910	2	6844	6	NULL	NULL	0	NULL	LDL	NULL	unlabeled	inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_14_8081_s_154	7713910	181 nM  unlabeled LDL inhibited  the binding of  I-LPL to LDL-coated plates by  approximately 50%  in both control and delipidated plates.	bind
24003	1	6845	5	13	NULL	NULL	NULL	luteinizing hormone beta gene	GP	rat	bind				upstream region	estrogen receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_941	11452016	184       Shupnik,M.A., Weinmann,C.M., Notides,A.C. and Chin,W.W. (1989) An upstream region of the rat luteinizing hormone beta gene binds estrogen receptor and confers estrogen responsiveness.	bind
24004	2	6845	5	13	NULL	NULL	NULL	luteinizing hormone beta gene	GP	rat	confers				upstream region	estrogen responsiveness	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_941	11452016	184       Shupnik,M.A., Weinmann,C.M., Notides,A.C. and Chin,W.W. (1989) An upstream region of the rat luteinizing hormone beta gene binds estrogen receptor and confers estrogen responsiveness.	bind
19911	1	6845	6	NULL	NULL	0	NULL	luteinizing hormone beta gene	NULL	rat	bind	NULL			upstream region	estrogen receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_941	11452016	184       Shupnik,M.A., Weinmann,C.M., Notides,A.C. and Chin,W.W. (1989) An upstream region of the rat luteinizing hormone beta gene binds estrogen receptor and confers estrogen responsiveness.	bind
19912	2	6845	6	NULL	NULL	0	NULL	statement 1	NULL		confers	NULL				estrogen responsiveness	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_941	11452016	184       Shupnik,M.A., Weinmann,C.M., Notides,A.C. and Chin,W.W. (1989) An upstream region of the rat luteinizing hormone beta gene binds estrogen receptor and confers estrogen responsiveness.	bind
24005	1	6847	5	13	NULL	NULL	NULL	platelet glycoprotein Ibbeta	GP	mutation in	results in				GATA binding site of promoter	Bernard-Soulier syndrome	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_1_312_s_182	11125123	19       Ludlow,L.B., Schick,B.P., Budarf,M.L., Driscoll,D.A., Zackai,E.H., Cohen,A. and Konkle,B.A. (1996) Identification of a mutation in a GATA binding site of the platelet glycoprotein Ibbeta promoter resulting in the Bernard-Soulier syndrome.	bind
19913	1	6847	6	NULL	NULL	0	NULL	platelet glycoprotein Ibbeta	NULL	mutant	results in	NULL			GATA binding site of the promoter	Bernard-Soulier syndrome	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_1_312_s_182	11125123	19       Ludlow,L.B., Schick,B.P., Budarf,M.L., Driscoll,D.A., Zackai,E.H., Cohen,A. and Konkle,B.A. (1996) Identification of a mutation in a GATA binding site of the platelet glycoprotein Ibbeta promoter resulting in the Bernard-Soulier syndrome.	bind
24006	1	6848	5	13	NULL	NULL	NULL	Ral 	GP		bind					GTP	Chemical	activated			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_899_s_32	11397694	19  Activated GTP-bound Ral binds to RLIP76 (or Ral binding protein), an effector molecule that possesses GTPase activity for cdc42 and Rac, suggesting a link between the activation of Ral and rearrangement of the cytoskeleton.	bind
24007	2	6848	5	13	NULL	NULL	NULL	statement 1	GP		bind					RLIP76	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_899_s_32	11397694	19  Activated GTP-bound Ral binds to RLIP76 (or Ral binding protein), an effector molecule that possesses GTPase activity for cdc42 and Rac, suggesting a link between the activation of Ral and rearrangement of the cytoskeleton.	bind
24008	3	6848	5	13	NULL	NULL	NULL	RLIP76	GP		possesses					cdc42 GTPase activity	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_899_s_32	11397694	19  Activated GTP-bound Ral binds to RLIP76 (or Ral binding protein), an effector molecule that possesses GTPase activity for cdc42 and Rac, suggesting a link between the activation of Ral and rearrangement of the cytoskeleton.	bind
24009	4	6848	5	13	NULL	NULL	NULL	RLIP76	GP		possesses					Rac GTPase activity	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_899_s_32	11397694	19  Activated GTP-bound Ral binds to RLIP76 (or Ral binding protein), an effector molecule that possesses GTPase activity for cdc42 and Rac, suggesting a link between the activation of Ral and rearrangement of the cytoskeleton.	bind
24010	5	6848	5	13	NULL	NULL	NULL	Ral	GP	activation of	is linked to					cytoskeleton	CellComponent	rearrangement of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_899_s_32	11397694	19  Activated GTP-bound Ral binds to RLIP76 (or Ral binding protein), an effector molecule that possesses GTPase activity for cdc42 and Rac, suggesting a link between the activation of Ral and rearrangement of the cytoskeleton.	bind
24011	6	6848	5	13	NULL	NULL	NULL	statement 3	Process		suggests					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_899_s_32	11397694	19  Activated GTP-bound Ral binds to RLIP76 (or Ral binding protein), an effector molecule that possesses GTPase activity for cdc42 and Rac, suggesting a link between the activation of Ral and rearrangement of the cytoskeleton.	bind
24012	7	6848	5	13	NULL	NULL	NULL	statement 4	Process		suggests					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_899_s_32	11397694	19  Activated GTP-bound Ral binds to RLIP76 (or Ral binding protein), an effector molecule that possesses GTPase activity for cdc42 and Rac, suggesting a link between the activation of Ral and rearrangement of the cytoskeleton.	bind
30351	8	6848	5	13	NULL	NULL	NULL	RLIP76	GP		is a type of					effector molecule	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_899_s_32	11397694	19  Activated GTP-bound Ral binds to RLIP76 (or Ral binding protein), an effector molecule that possesses GTPase activity for cdc42 and Rac, suggesting a link between the activation of Ral and rearrangement of the cytoskeleton.	bind
56630	9	6848	5	13	NULL	NULL	NULL	RLIP76	GP		is a type of					Ral binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_899_s_32	11397694	19  Activated GTP-bound Ral binds to RLIP76 (or Ral binding protein), an effector molecule that possesses GTPase activity for cdc42 and Rac, suggesting a link between the activation of Ral and rearrangement of the cytoskeleton.	bind
19914	1	6848	6	NULL	NULL	0	NULL	Ral	NULL		bind	NULL				GTP	NULL	activated			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_899_s_32	11397694	19  Activated GTP-bound Ral binds to RLIP76 (or Ral binding protein), an effector molecule that possesses GTPase activity for cdc42 and Rac, suggesting a link between the activation of Ral and rearrangement of the cytoskeleton.	bind
19915	2	6848	6	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL				RLIP76	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_899_s_32	11397694	19  Activated GTP-bound Ral binds to RLIP76 (or Ral binding protein), an effector molecule that possesses GTPase activity for cdc42 and Rac, suggesting a link between the activation of Ral and rearrangement of the cytoskeleton.	bind
19916	3	6848	6	NULL	NULL	0	NULL	RLIP76	NULL		is a type of	NULL				Ral binding protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_899_s_32	11397694	19  Activated GTP-bound Ral binds to RLIP76 (or Ral binding protein), an effector molecule that possesses GTPase activity for cdc42 and Rac, suggesting a link between the activation of Ral and rearrangement of the cytoskeleton.	bind
19917	4	6848	6	NULL	NULL	0	NULL	RLIP76	NULL		possesses	NULL				GTPase activity	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_899_s_32	11397694	19  Activated GTP-bound Ral binds to RLIP76 (or Ral binding protein), an effector molecule that possesses GTPase activity for cdc42 and Rac, suggesting a link between the activation of Ral and rearrangement of the cytoskeleton.	bind
19918	5	6848	6	NULL	NULL	0	NULL	statement 4	NULL		occurs for	NULL				cdc42 GTPase activity	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_899_s_32	11397694	19  Activated GTP-bound Ral binds to RLIP76 (or Ral binding protein), an effector molecule that possesses GTPase activity for cdc42 and Rac, suggesting a link between the activation of Ral and rearrangement of the cytoskeleton.	bind
19919	6	6848	6	NULL	NULL	0	NULL	statement 4	NULL		occurs for	NULL				Rac GTPase activity	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_899_s_32	11397694	19  Activated GTP-bound Ral binds to RLIP76 (or Ral binding protein), an effector molecule that possesses GTPase activity for cdc42 and Rac, suggesting a link between the activation of Ral and rearrangement of the cytoskeleton.	bind
30288	7	6848	6	NULL	NULL	0	NULL	RLIP76	NULL		is a type of	NULL				effector molecule	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_899_s_32	11397694	19  Activated GTP-bound Ral binds to RLIP76 (or Ral binding protein), an effector molecule that possesses GTPase activity for cdc42 and Rac, suggesting a link between the activation of Ral and rearrangement of the cytoskeleton.	bind
56631	8	6848	6	10	NULL	0	NULL	Ral		activation of	is linked to					cytoskeleton		rearrangement of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_899_s_32	11397694	19  Activated GTP-bound Ral binds to RLIP76 (or Ral binding protein), an effector molecule that possesses GTPase activity for cdc42 and Rac, suggesting a link between the activation of Ral and rearrangement of the cytoskeleton.	bind
56632	9	6848	6	10	NULL	0	NULL	statement 5			suggests					statement 8					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_899_s_32	11397694	19  Activated GTP-bound Ral binds to RLIP76 (or Ral binding protein), an effector molecule that possesses GTPase activity for cdc42 and Rac, suggesting a link between the activation of Ral and rearrangement of the cytoskeleton.	bind
56633	10	6848	6	10	NULL	0	NULL	statement 6			suggests					statement 8					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_899_s_32	11397694	19  Activated GTP-bound Ral binds to RLIP76 (or Ral binding protein), an effector molecule that possesses GTPase activity for cdc42 and Rac, suggesting a link between the activation of Ral and rearrangement of the cytoskeleton.	bind
30352	1	6849	5	13	NULL	NULL	NULL	TNF-alpha	GP		bind					55kd membrane receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_6_1839_s_180	9846974	19  As a trimeric complex, TNF-alpha binds to the two demonstrated membrane receptors of 55kd and 75kd.	bind
30353	2	6849	5	13	NULL	NULL	NULL	TNF-alpha	GP		bind					75kd membrane receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_6_1839_s_180	9846974	19  As a trimeric complex, TNF-alpha binds to the two demonstrated membrane receptors of 55kd and 75kd.	bind
30354	3	6849	5	13	NULL	NULL	NULL	statement 1	GP		forms complex with					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_6_1839_s_180	9846974	19  As a trimeric complex, TNF-alpha binds to the two demonstrated membrane receptors of 55kd and 75kd.	bind
19920	1	6849	6	NULL	NULL	0	NULL	TNF-alpha	NULL		bind	NULL				55kd membrane receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_6_1839_s_180	9846974	19  As a trimeric complex, TNF-alpha binds to the two demonstrated membrane receptors of 55kd and 75kd.	bind
19921	2	6849	6	NULL	NULL	0	NULL	TNF-alpha	NULL		bind	NULL				75kd membrane receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_6_1839_s_180	9846974	19  As a trimeric complex, TNF-alpha binds to the two demonstrated membrane receptors of 55kd and 75kd.	bind
19922	3	6849	6	NULL	NULL	0	NULL	statement 1	NULL		forms complex with	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_6_1839_s_180	9846974	19  As a trimeric complex, TNF-alpha binds to the two demonstrated membrane receptors of 55kd and 75kd.	bind
24014	1	6850	5	13	NULL	NULL	NULL	CKIs	GP		bind					CDK  complexes	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_1_119_s_18	9916926	19  CKIs bind to cyclin/cyclin-dependent kinase (CDK) complexes, consequently blocking progression through the cell cycle.	bind
24015	2	6850	5	13	NULL	NULL	NULL	CDK  complexes	GP		is					cyclin/cyclin-dependent kinase complexes	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_1_119_s_18	9916926	19  CKIs bind to cyclin/cyclin-dependent kinase (CDK) complexes, consequently blocking progression through the cell cycle.	bind
24016	3	6850	5	13	NULL	NULL	NULL	statement 1	Process		blocks					cell cycle	Process	progression through			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_1_119_s_18	9916926	19  CKIs bind to cyclin/cyclin-dependent kinase (CDK) complexes, consequently blocking progression through the cell cycle.	bind
19923	1	6850	6	NULL	NULL	0	NULL	CKI	NULL		bind	NULL				CDK complexes	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_1_119_s_18	9916926	19  CKIs bind to cyclin/cyclin-dependent kinase (CDK) complexes, consequently blocking progression through the cell cycle.	bind
19924	2	6850	6	NULL	NULL	0	NULL	CDK	NULL		is	NULL				cyclin/cyclin-dependent kinase	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_1_119_s_18	9916926	19  CKIs bind to cyclin/cyclin-dependent kinase (CDK) complexes, consequently blocking progression through the cell cycle.	bind
30289	3	6850	6	NULL	NULL	0	NULL	statement 1	NULL		blocks	NULL				cell cycle	NULL	progression through			NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_1_119_s_18	9916926	19  CKIs bind to cyclin/cyclin-dependent kinase (CDK) complexes, consequently blocking progression through the cell cycle.	bind
24017	1	6851	5	13	NULL	NULL	NULL	angiotensin II	GP		bind					AT1 receptors	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulation_103_6_904_s_72	11171802	19  In vitro, losartan competes with the binding of angiotensin II to AT1 receptors; the concentration that inhibits 50% of the binding of angiotensin II (IC50) is 20 nmol/L. Losartan has a major active metabolite, EXP 3174.	bind
24018	2	6851	5	13	NULL	NULL	NULL	losartan	Chemical		bind					AT1 receptors	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulation_103_6_904_s_72	11171802	19  In vitro, losartan competes with the binding of angiotensin II to AT1 receptors; the concentration that inhibits 50% of the binding of angiotensin II (IC50) is 20 nmol/L. Losartan has a major active metabolite, EXP 3174.	bind
24019	3	6851	5	13	NULL	NULL	NULL	statement 2	Process		competes with					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulation_103_6_904_s_72	11171802	19  In vitro, losartan competes with the binding of angiotensin II to AT1 receptors; the concentration that inhibits 50% of the binding of angiotensin II (IC50) is 20 nmol/L. Losartan has a major active metabolite, EXP 3174.	bind
24020	4	6851	5	13	NULL	NULL	NULL	EXP 3174	Chemical		is a metabolite of		major active			losartan	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_6_904_s_72	11171802	19  In vitro, losartan competes with the binding of angiotensin II to AT1 receptors; the concentration that inhibits 50% of the binding of angiotensin II (IC50) is 20 nmol/L. Losartan has a major active metabolite, EXP 3174.	bind
19925	1	6851	6	NULL	NULL	0	NULL	angiotensin II	NULL		bind	NULL				AT1 receptor	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulation_103_6_904_s_72	11171802	19  In vitro, losartan competes with the binding of angiotensin II to AT1 receptors; the concentration that inhibits 50% of the binding of angiotensin II (IC50) is 20 nmol/L. Losartan has a major active metabolite, EXP 3174.	bind
19926	2	6851	6	NULL	NULL	0	NULL	losartan	NULL		bind	NULL				AT1 receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_6_904_s_72	11171802	19  In vitro, losartan competes with the binding of angiotensin II to AT1 receptors; the concentration that inhibits 50% of the binding of angiotensin II (IC50) is 20 nmol/L. Losartan has a major active metabolite, EXP 3174.	bind
19927	3	6851	6	NULL	NULL	0	NULL	statement 1	NULL		competes	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_6_904_s_72	11171802	19  In vitro, losartan competes with the binding of angiotensin II to AT1 receptors; the concentration that inhibits 50% of the binding of angiotensin II (IC50) is 20 nmol/L. Losartan has a major active metabolite, EXP 3174.	bind
19932	4	6851	6	NULL	NULL	0	NULL	EXP 3174	NULL		is an active metabolite for	NULL				Losartan	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_6_904_s_72	11171802	19  In vitro, losartan competes with the binding of angiotensin II to AT1 receptors; the concentration that inhibits 50% of the binding of angiotensin II (IC50) is 20 nmol/L. Losartan has a major active metabolite, EXP 3174.	bind
24243	1	6852	5	13	NULL	NULL	NULL	Ang-2	GP		is antagonist of					Ang-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_6_2077_s_252	10854229	19  It has been proposed that Ang-2, the Ang-1 antagonist that binds to Tie-2 and blocks Ang-1-induced Tie-2 phosphorylation, could be an important pro-angiogenic factor, in that by interrupting the stabilizing Ang-1 signal it might promote a process of vessel wall disassembly that would allow endothelial cells to respond to angiogenic inducers.	bind
24244	2	6852	5	13	NULL	NULL	NULL	Ang-2	GP		bind					Tie-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_6_2077_s_252	10854229	19  It has been proposed that Ang-2, the Ang-1 antagonist that binds to Tie-2 and blocks Ang-1-induced Tie-2 phosphorylation, could be an important pro-angiogenic factor, in that by interrupting the stabilizing Ang-1 signal it might promote a process of vessel wall disassembly that would allow endothelial cells to respond to angiogenic inducers.	bind
24245	3	6852	5	13	NULL	NULL	NULL	Ang-1	GP		induces					Tie-2	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_6_2077_s_252	10854229	19  It has been proposed that Ang-2, the Ang-1 antagonist that binds to Tie-2 and blocks Ang-1-induced Tie-2 phosphorylation, could be an important pro-angiogenic factor, in that by interrupting the stabilizing Ang-1 signal it might promote a process of vessel wall disassembly that would allow endothelial cells to respond to angiogenic inducers.	bind
24246	4	6852	5	13	NULL	NULL	NULL	statement 2	Process		blocks					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_6_2077_s_252	10854229	19  It has been proposed that Ang-2, the Ang-1 antagonist that binds to Tie-2 and blocks Ang-1-induced Tie-2 phosphorylation, could be an important pro-angiogenic factor, in that by interrupting the stabilizing Ang-1 signal it might promote a process of vessel wall disassembly that would allow endothelial cells to respond to angiogenic inducers.	bind
24247	5	6852	5	13	NULL	NULL	NULL	Ang-2	GP		interrupts					Ang-1	GP	stabilizing signal of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_6_2077_s_252	10854229	19  It has been proposed that Ang-2, the Ang-1 antagonist that binds to Tie-2 and blocks Ang-1-induced Tie-2 phosphorylation, could be an important pro-angiogenic factor, in that by interrupting the stabilizing Ang-1 signal it might promote a process of vessel wall disassembly that would allow endothelial cells to respond to angiogenic inducers.	bind
24248	6	6852	5	13	NULL	NULL	NULL	statement 5	Process		promote		might			vessel wall disassembly	Process	process of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_6_2077_s_252	10854229	19  It has been proposed that Ang-2, the Ang-1 antagonist that binds to Tie-2 and blocks Ang-1-induced Tie-2 phosphorylation, could be an important pro-angiogenic factor, in that by interrupting the stabilizing Ang-1 signal it might promote a process of vessel wall disassembly that would allow endothelial cells to respond to angiogenic inducers.	bind
24249	7	6852	5	13	NULL	NULL	NULL	endothelial cells	Cell		responds to					angiogenic inducers	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_6_2077_s_252	10854229	19  It has been proposed that Ang-2, the Ang-1 antagonist that binds to Tie-2 and blocks Ang-1-induced Tie-2 phosphorylation, could be an important pro-angiogenic factor, in that by interrupting the stabilizing Ang-1 signal it might promote a process of vessel wall disassembly that would allow endothelial cells to respond to angiogenic inducers.	bind
24250	8	6852	5	13	NULL	NULL	NULL	statement 6	Process		allows					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_6_2077_s_252	10854229	19  It has been proposed that Ang-2, the Ang-1 antagonist that binds to Tie-2 and blocks Ang-1-induced Tie-2 phosphorylation, could be an important pro-angiogenic factor, in that by interrupting the stabilizing Ang-1 signal it might promote a process of vessel wall disassembly that would allow endothelial cells to respond to angiogenic inducers.	bind
24251	9	6852	5	13	NULL	NULL	NULL	Ang-2	GP		is a type of					pro-angiogenic factor	GP	 important			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_6_2077_s_252	10854229	19  It has been proposed that Ang-2, the Ang-1 antagonist that binds to Tie-2 and blocks Ang-1-induced Tie-2 phosphorylation, could be an important pro-angiogenic factor, in that by interrupting the stabilizing Ang-1 signal it might promote a process of vessel wall disassembly that would allow endothelial cells to respond to angiogenic inducers.	bind
19935	1	6852	6	NULL	NULL	0	NULL	Ang-2	NULL		bind	NULL				Tie-2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_6_2077_s_252	10854229	19  It has been proposed that Ang-2, the Ang-1 antagonist that binds to Tie-2 and blocks Ang-1-induced Tie-2 phosphorylation, could be an important pro-angiogenic factor, in that by interrupting the stabilizing Ang-1 signal it might promote a process of vessel wall disassembly that would allow endothelial cells to respond to angiogenic inducers.	bind
19971	2	6852	6	10	NULL	0	NULL	Ang-2			is antagonist of					Ang-1					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_6_2077_s_252	10854229	19  It has been proposed that Ang-2, the Ang-1 antagonist that binds to Tie-2 and blocks Ang-1-induced Tie-2 phosphorylation, could be an important pro-angiogenic factor, in that by interrupting the stabilizing Ang-1 signal it might promote a process of vessel wall disassembly that would allow endothelial cells to respond to angiogenic inducers.	bind
19972	3	6852	6	NULL	NULL	0	NULL	Ang-1	NULL		induces	NULL				Tie-2	NULL	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_6_2077_s_252	10854229	19  It has been proposed that Ang-2, the Ang-1 antagonist that binds to Tie-2 and blocks Ang-1-induced Tie-2 phosphorylation, could be an important pro-angiogenic factor, in that by interrupting the stabilizing Ang-1 signal it might promote a process of vessel wall disassembly that would allow endothelial cells to respond to angiogenic inducers.	bind
19973	4	6852	6	NULL	NULL	0	NULL	Ang-2	NULL		blocks	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_6_2077_s_252	10854229	19  It has been proposed that Ang-2, the Ang-1 antagonist that binds to Tie-2 and blocks Ang-1-induced Tie-2 phosphorylation, could be an important pro-angiogenic factor, in that by interrupting the stabilizing Ang-1 signal it might promote a process of vessel wall disassembly that would allow endothelial cells to respond to angiogenic inducers.	bind
19974	5	6852	6	10	NULL	0	NULL	Ang-2			is a type of					pro-angiogenic factor					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_6_2077_s_252	10854229	19  It has been proposed that Ang-2, the Ang-1 antagonist that binds to Tie-2 and blocks Ang-1-induced Tie-2 phosphorylation, could be an important pro-angiogenic factor, in that by interrupting the stabilizing Ang-1 signal it might promote a process of vessel wall disassembly that would allow endothelial cells to respond to angiogenic inducers.	bind
19975	6	6852	6	NULL	NULL	0	NULL	Ang-2	NULL		promote	NULL	might			vessel wall disassembly	NULL	process of 			NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_6_2077_s_252	10854229	19  It has been proposed that Ang-2, the Ang-1 antagonist that binds to Tie-2 and blocks Ang-1-induced Tie-2 phosphorylation, could be an important pro-angiogenic factor, in that by interrupting the stabilizing Ang-1 signal it might promote a process of vessel wall disassembly that would allow endothelial cells to respond to angiogenic inducers.	bind
19976	7	6852	6	NULL	NULL	0	NULL	endothelial cells	NULL		respond to	NULL				angiogenic inducers	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_6_2077_s_252	10854229	19  It has been proposed that Ang-2, the Ang-1 antagonist that binds to Tie-2 and blocks Ang-1-induced Tie-2 phosphorylation, could be an important pro-angiogenic factor, in that by interrupting the stabilizing Ang-1 signal it might promote a process of vessel wall disassembly that would allow endothelial cells to respond to angiogenic inducers.	bind
19977	8	6852	6	NULL	NULL	0	NULL	statement 6	NULL		allow	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_6_2077_s_252	10854229	19  It has been proposed that Ang-2, the Ang-1 antagonist that binds to Tie-2 and blocks Ang-1-induced Tie-2 phosphorylation, could be an important pro-angiogenic factor, in that by interrupting the stabilizing Ang-1 signal it might promote a process of vessel wall disassembly that would allow endothelial cells to respond to angiogenic inducers.	bind
56634	9	6852	6	10	NULL	0	NULL	Ang-2			interrupts 					Ang-1		stabilizing signal of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_6_2077_s_252	10854229	19  It has been proposed that Ang-2, the Ang-1 antagonist that binds to Tie-2 and blocks Ang-1-induced Tie-2 phosphorylation, could be an important pro-angiogenic factor, in that by interrupting the stabilizing Ang-1 signal it might promote a process of vessel wall disassembly that would allow endothelial cells to respond to angiogenic inducers.	bind
56635	1	6853	5	13	NULL	NULL	NULL	actin monomer-binding proteins	GP		bind					 monomeric actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_869_s_258	11891186	19  They were then identified as actin monomer-binding proteins 20, 21  that bind monomeric actin (G-actin) and disturb the assembly of filamentous actin (F-actin).	bind
56636	2	6853	5	13	NULL	NULL	NULL	actin monomer-binding proteins	GP		disturb					filamentous actin	GP	 assembly of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_869_s_258	11891186	19  They were then identified as actin monomer-binding proteins 20, 21  that bind monomeric actin (G-actin) and disturb the assembly of filamentous actin (F-actin).	bind
56637	3	6853	5	13	NULL	NULL	NULL	G-actin	GP		is a type of					monomeric actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_869_s_258	11891186	19  They were then identified as actin monomer-binding proteins 20, 21  that bind monomeric actin (G-actin) and disturb the assembly of filamentous actin (F-actin).	bind
56638	4	6853	5	13	NULL	NULL	NULL	F-actin	GP		is a type of					filamentous actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_869_s_258	11891186	19  They were then identified as actin monomer-binding proteins 20, 21  that bind monomeric actin (G-actin) and disturb the assembly of filamentous actin (F-actin).	bind
19978	1	6853	6	NULL	NULL	0	NULL	actin monomer-binding proteins	NULL		bind	NULL				monomeric actin	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_3_869_s_258	11891186	19  They were then identified as actin monomer-binding proteins 20, 21  that bind monomeric actin (G-actin) and disturb the assembly of filamentous actin (F-actin).	bind
19979	2	6853	6	NULL	NULL	0	NULL	actin monomer-binding proteins	NULL		disturb	NULL				filamentous actin	NULL	assembly of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_3_869_s_258	11891186	19  They were then identified as actin monomer-binding proteins 20, 21  that bind monomeric actin (G-actin) and disturb the assembly of filamentous actin (F-actin).	bind
19980	3	6853	6	10	NULL	0	NULL	G-actin	NULL		is a type of	NULL				monomeric actin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_869_s_258	11891186	19  They were then identified as actin monomer-binding proteins 20, 21  that bind monomeric actin (G-actin) and disturb the assembly of filamentous actin (F-actin).	bind
19981	4	6853	6	10	NULL	0	NULL	F-actin	NULL		is a type of	NULL				filamentous actin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_869_s_258	11891186	19  They were then identified as actin monomer-binding proteins 20, 21  that bind monomeric actin (G-actin) and disturb the assembly of filamentous actin (F-actin).	bind
24252	1	6854	5	13	NULL	NULL	NULL	Tie-2	GP		is					 receptor tyrosine kinase	GP	endothelium-specific			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_3_799_s_144	12213707	19  Tie-2 is an endothelium-specific receptor tyrosine kinase, which binds to angiopoietin-1 and -2.	bind
24253	2	6854	5	13	NULL	NULL	NULL	Tie-2	GP		bind					angiopoietin-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_3_799_s_144	12213707	19  Tie-2 is an endothelium-specific receptor tyrosine kinase, which binds to angiopoietin-1 and -2.	bind
24254	3	6854	5	13	NULL	NULL	NULL	Tie-2	GP		bind					angiopoietin-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_3_799_s_144	12213707	19  Tie-2 is an endothelium-specific receptor tyrosine kinase, which binds to angiopoietin-1 and -2.	bind
19982	1	6854	6	NULL	NULL	0	NULL	Tie-2	NULL		bind	NULL				angiopoietin-1	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_3_799_s_144	12213707	19  Tie-2 is an endothelium-specific receptor tyrosine kinase, which binds to angiopoietin-1 and -2.	bind
19983	2	6854	6	NULL	NULL	0	NULL	Tie-2	NULL		bind	NULL				angiopoietin-2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_3_799_s_144	12213707	19  Tie-2 is an endothelium-specific receptor tyrosine kinase, which binds to angiopoietin-1 and -2.	bind
19985	3	6854	6	NULL	NULL	0	NULL	Tie-2	NULL		is	NULL				receptor tyrosine kinase	NULL	endothelium specific			NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_3_799_s_144	12213707	19  Tie-2 is an endothelium-specific receptor tyrosine kinase, which binds to angiopoietin-1 and -2.	bind
24255	1	6855	5	13	NULL	NULL	NULL	monocytes	Cell	human	express					FcRgammaIIa	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_975_s_36	15044210	19 - 22    Human monocytes express FcRgammaIIa or CD32, which binds CRP with high affinity and has been described as putative CRP-receptor 23 and FcRgammaI or CD64, which binds CRP with lower affinity.	bind
24256	2	6855	5	13	NULL	NULL	NULL	FcRgammaIIa 	GP		is					CD32	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_975_s_36	15044210	19 - 22    Human monocytes express FcRgammaIIa or CD32, which binds CRP with high affinity and has been described as putative CRP-receptor 23 and FcRgammaI or CD64, which binds CRP with lower affinity.	bind
24258	3	6855	5	13	NULL	NULL	NULL	FcRgammaIIa	GP		bind		high affinity			CRP	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_975_s_36	15044210	19 - 22    Human monocytes express FcRgammaIIa or CD32, which binds CRP with high affinity and has been described as putative CRP-receptor 23 and FcRgammaI or CD64, which binds CRP with lower affinity.	bind
24259	5	6855	5	13	NULL	NULL	NULL	FcRgammaIIa	GP		is described as					CRP-receptor	GP	putative			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_975_s_36	15044210	19 - 22    Human monocytes express FcRgammaIIa or CD32, which binds CRP with high affinity and has been described as putative CRP-receptor 23 and FcRgammaI or CD64, which binds CRP with lower affinity.	bind
24260	6	6855	5	13	NULL	NULL	NULL	monocytes	Cell	human	express					FcRgammaI	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_975_s_36	15044210	19 - 22    Human monocytes express FcRgammaIIa or CD32, which binds CRP with high affinity and has been described as putative CRP-receptor 23 and FcRgammaI or CD64, which binds CRP with lower affinity.	bind
24261	7	6855	5	13	NULL	NULL	NULL	FcRgammaI	GP		is					CD64	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_975_s_36	15044210	19 - 22    Human monocytes express FcRgammaIIa or CD32, which binds CRP with high affinity and has been described as putative CRP-receptor 23 and FcRgammaI or CD64, which binds CRP with lower affinity.	bind
24262	4	6855	5	13	NULL	NULL	NULL	FcRgammaI	GP		bind		low affinity			CRP	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_975_s_36	15044210	19 - 22    Human monocytes express FcRgammaIIa or CD32, which binds CRP with high affinity and has been described as putative CRP-receptor 23 and FcRgammaI or CD64, which binds CRP with lower affinity.	bind
19986	1	6855	6	NULL	NULL	0	NULL	monocytes	NULL	human	express	NULL				FcRgammaIIa	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_975_s_36	15044210	19 - 22    Human monocytes express FcRgammaIIa or CD32, which binds CRP with high affinity and has been described as putative CRP-receptor 23 and FcRgammaI or CD64, which binds CRP with lower affinity.	bind
19988	2	6855	6	NULL	NULL	0	NULL	FcRgammaIIa	NULL		is	NULL				CD32	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_975_s_36	15044210	19 - 22    Human monocytes express FcRgammaIIa or CD32, which binds CRP with high affinity and has been described as putative CRP-receptor 23 and FcRgammaI or CD64, which binds CRP with lower affinity.	bind
19989	3	6855	6	NULL	NULL	0	NULL	FcRgammaIIa	NULL		bind	NULL	high affinity			CRP	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_975_s_36	15044210	19 - 22    Human monocytes express FcRgammaIIa or CD32, which binds CRP with high affinity and has been described as putative CRP-receptor 23 and FcRgammaI or CD64, which binds CRP with lower affinity.	bind
20295	4	6855	6	10	NULL	0	NULL	FcRgammaIIa			is described as					 CRP-receptor		putative			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_975_s_36	15044210	19 - 22    Human monocytes express FcRgammaIIa or CD32, which binds CRP with high affinity and has been described as putative CRP-receptor 23 and FcRgammaI or CD64, which binds CRP with lower affinity.	bind
20296	5	6855	6	NULL	NULL	0	NULL	FcRgammaI	NULL		bind	NULL	low affinity			CRP	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_975_s_36	15044210	19 - 22    Human monocytes express FcRgammaIIa or CD32, which binds CRP with high affinity and has been described as putative CRP-receptor 23 and FcRgammaI or CD64, which binds CRP with lower affinity.	bind
20297	6	6855	6	NULL	NULL	0	NULL	FcRgammaI	NULL		is	NULL				CD64	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_975_s_36	15044210	19 - 22    Human monocytes express FcRgammaIIa or CD32, which binds CRP with high affinity and has been described as putative CRP-receptor 23 and FcRgammaI or CD64, which binds CRP with lower affinity.	bind
56639	7	6855	6	10	NULL	0	NULL	monocytes		human	express					FcRgammaI					NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_975_s_36	15044210	19 - 22    Human monocytes express FcRgammaIIa or CD32, which binds CRP with high affinity and has been described as putative CRP-receptor 23 and FcRgammaI or CD64, which binds CRP with lower affinity.	bind
24263	1	6856	5	13	NULL	NULL	NULL	egr-1	GP	activated	bind					PDGF-A	GP	proximal		promoter	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_4_996_s_36	10195928	19 20  Activated  egr-1 binds to the proximal PDGF-A promoter by displacing  sp-1 from their overlapping recognition element, and the  egr-1 binding site has been identified as a cis-element for the induction of PDGF-A by fluid shear.	bind
24264	2	6856	5	13	NULL	NULL	NULL	sp-1	GP		is displaced from							overlapping		recognition element	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_4_996_s_36	10195928	19 20  Activated  egr-1 binds to the proximal PDGF-A promoter by displacing  sp-1 from their overlapping recognition element, and the  egr-1 binding site has been identified as a cis-element for the induction of PDGF-A by fluid shear.	bind
24265	3	6856	5	13	NULL	NULL	NULL	statement 1	Process		occurs by					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_4_996_s_36	10195928	19 20  Activated  egr-1 binds to the proximal PDGF-A promoter by displacing  sp-1 from their overlapping recognition element, and the  egr-1 binding site has been identified as a cis-element for the induction of PDGF-A by fluid shear.	bind
24266	5	6856	5	NULL	NULL	0	NULL		NULL		has been identified as	NULL			egr-1 binding site		NULL			cis-element	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_4_996_s_36	10195928	19 20  Activated  egr-1 binds to the proximal PDGF-A promoter by displacing  sp-1 from their overlapping recognition element, and the  egr-1 binding site has been identified as a cis-element for the induction of PDGF-A by fluid shear.	bind
24267	4	6856	5	13	NULL	NULL	NULL	PDGF-A	GP		is induced by					fluid shear					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_4_996_s_36	10195928	19 20  Activated  egr-1 binds to the proximal PDGF-A promoter by displacing  sp-1 from their overlapping recognition element, and the  egr-1 binding site has been identified as a cis-element for the induction of PDGF-A by fluid shear.	bind
24268	6	6856	5	13	NULL	NULL	NULL	statement 5	Process		is required for					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_4_996_s_36	10195928	19 20  Activated  egr-1 binds to the proximal PDGF-A promoter by displacing  sp-1 from their overlapping recognition element, and the  egr-1 binding site has been identified as a cis-element for the induction of PDGF-A by fluid shear.	bind
19990	1	6856	6	NULL	NULL	0	NULL	egr-1	NULL	activated	bind	NULL				PDGF-A	NULL	proximal		promoter	NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_4_996_s_36	10195928	19 20  Activated  egr-1 binds to the proximal PDGF-A promoter by displacing  sp-1 from their overlapping recognition element, and the  egr-1 binding site has been identified as a cis-element for the induction of PDGF-A by fluid shear.	bind
19991	2	6856	6	NULL	NULL	0	NULL		NULL		induces	NULL			egr-1 binding site	PDGF-A	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_4_996_s_36	10195928	19 20  Activated  egr-1 binds to the proximal PDGF-A promoter by displacing  sp-1 from their overlapping recognition element, and the  egr-1 binding site has been identified as a cis-element for the induction of PDGF-A by fluid shear.	bind
19992	3	6856	6	NULL	NULL	0	NULL	statement 2	NULL		occurs by	NULL				fluid shear	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_4_996_s_36	10195928	19 20  Activated  egr-1 binds to the proximal PDGF-A promoter by displacing  sp-1 from their overlapping recognition element, and the  egr-1 binding site has been identified as a cis-element for the induction of PDGF-A by fluid shear.	bind
20757	4	6856	6	NULL	NULL	0	NULL	egr-1	NULL		displaces	NULL				Sp1	NULL	overlapping 		recognition element	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_4_996_s_36	10195928	19 20  Activated  egr-1 binds to the proximal PDGF-A promoter by displacing  sp-1 from their overlapping recognition element, and the  egr-1 binding site has been identified as a cis-element for the induction of PDGF-A by fluid shear.	bind
20758	5	6856	6	NULL	NULL	0	NULL	statement 1	NULL		occurs by	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_4_996_s_36	10195928	19 20  Activated  egr-1 binds to the proximal PDGF-A promoter by displacing  sp-1 from their overlapping recognition element, and the  egr-1 binding site has been identified as a cis-element for the induction of PDGF-A by fluid shear.	bind
56640	6	6856	6	10	NULL	0	NULL				has been identified as			 egr-1 binding site						cis-element	NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_4_996_s_36	10195928	19 20  Activated  egr-1 binds to the proximal PDGF-A promoter by displacing  sp-1 from their overlapping recognition element, and the  egr-1 binding site has been identified as a cis-element for the induction of PDGF-A by fluid shear.	bind
24269	1	6858	5	13	NULL	NULL	NULL	TF	GP		is a type of					integral membrane glycoprotein	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_3_520_s_35	9102171	19 22  TF is an integral membrane glycoprotein, which binds to factor VII(a).	bind
24270	2	6858	5	13	NULL	NULL	NULL	TF	GP		bind					factor VII	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_3_520_s_35	9102171	19 22  TF is an integral membrane glycoprotein, which binds to factor VII(a).	bind
19995	1	6858	6	NULL	NULL	0	NULL	TF	NULL		bind	NULL				factor VII	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_3_520_s_35	9102171	19 22  TF is an integral membrane glycoprotein, which binds to factor VII(a).	bind
19996	2	6858	6	10	NULL	0	NULL	TF	NULL		is a type of	NULL				integral membrane glycoprotein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_3_520_s_35	9102171	19 22  TF is an integral membrane glycoprotein, which binds to factor VII(a).	bind
24271	1	6859	5	13	NULL	NULL	NULL	Hdlq19 gene	GP		code for		may			plasma phospholipid transfer protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_161_s_133	14592847	19 A candidate gene for  Hdlq19 is the gene ( Pltp; cM 93.0) coding for plasma phospholipid transfer protein, which is bound to HDL and mediates the net transfer and exchange of phospholipids among different lipoproteins and participates in the transformation of larger HDL3 into smaller HDL2.	bind
24272	2	6859	5	13	NULL	NULL	NULL	statement 1	GP		bind					HDL	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_161_s_133	14592847	19 A candidate gene for  Hdlq19 is the gene ( Pltp; cM 93.0) coding for plasma phospholipid transfer protein, which is bound to HDL and mediates the net transfer and exchange of phospholipids among different lipoproteins and participates in the transformation of larger HDL3 into smaller HDL2.	bind
24273	3	6859	5	13	NULL	NULL	NULL	statement 2	Process		mediate					phospholipids	Chemical	net transfer of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_161_s_133	14592847	19 A candidate gene for  Hdlq19 is the gene ( Pltp; cM 93.0) coding for plasma phospholipid transfer protein, which is bound to HDL and mediates the net transfer and exchange of phospholipids among different lipoproteins and participates in the transformation of larger HDL3 into smaller HDL2.	bind
24274	4	6859	5	13	NULL	NULL	NULL	statement 2	Process		mediate					phospholipids	Chemical	exchange of 			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_161_s_133	14592847	19 A candidate gene for  Hdlq19 is the gene ( Pltp; cM 93.0) coding for plasma phospholipid transfer protein, which is bound to HDL and mediates the net transfer and exchange of phospholipids among different lipoproteins and participates in the transformation of larger HDL3 into smaller HDL2.	bind
24275	5	6859	5	13	NULL	NULL	NULL	HDL3	GP	larger	is transformed to					HDL2	GP	smaller			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_161_s_133	14592847	19 A candidate gene for  Hdlq19 is the gene ( Pltp; cM 93.0) coding for plasma phospholipid transfer protein, which is bound to HDL and mediates the net transfer and exchange of phospholipids among different lipoproteins and participates in the transformation of larger HDL3 into smaller HDL2.	bind
24276	6	6859	5	13	NULL	NULL	NULL	statement 2	Process		participates in					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_161_s_133	14592847	19 A candidate gene for  Hdlq19 is the gene ( Pltp; cM 93.0) coding for plasma phospholipid transfer protein, which is bound to HDL and mediates the net transfer and exchange of phospholipids among different lipoproteins and participates in the transformation of larger HDL3 into smaller HDL2.	bind
19997	1	6859	6	NULL	NULL	0	NULL	Hdlq19 gene	NULL		codes for	NULL				plasma phospholipid transfer protein	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_161_s_133	14592847	19 A candidate gene for  Hdlq19 is the gene ( Pltp; cM 93.0) coding for plasma phospholipid transfer protein, which is bound to HDL and mediates the net transfer and exchange of phospholipids among different lipoproteins and participates in the transformation of larger HDL3 into smaller HDL2.	bind
19998	2	6859	6	NULL	NULL	0	NULL	plasma phospholipid transfer protein	NULL		bind	NULL				HDL	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_161_s_133	14592847	19 A candidate gene for  Hdlq19 is the gene ( Pltp; cM 93.0) coding for plasma phospholipid transfer protein, which is bound to HDL and mediates the net transfer and exchange of phospholipids among different lipoproteins and participates in the transformation of larger HDL3 into smaller HDL2.	bind
19999	3	6859	6	NULL	NULL	0	NULL	statement 2	NULL		mediates	NULL				phospholipids	NULL	transfer of 			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_161_s_133	14592847	19 A candidate gene for  Hdlq19 is the gene ( Pltp; cM 93.0) coding for plasma phospholipid transfer protein, which is bound to HDL and mediates the net transfer and exchange of phospholipids among different lipoproteins and participates in the transformation of larger HDL3 into smaller HDL2.	bind
20000	4	6859	6	NULL	NULL	0	NULL	statement 2	NULL		mediates	NULL				phospholipids	NULL	exchange of 			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_161_s_133	14592847	19 A candidate gene for  Hdlq19 is the gene ( Pltp; cM 93.0) coding for plasma phospholipid transfer protein, which is bound to HDL and mediates the net transfer and exchange of phospholipids among different lipoproteins and participates in the transformation of larger HDL3 into smaller HDL2.	bind
20001	5	6859	6	NULL	NULL	0	NULL	HDL3	NULL		transformed into	NULL				HDL2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_161_s_133	14592847	19 A candidate gene for  Hdlq19 is the gene ( Pltp; cM 93.0) coding for plasma phospholipid transfer protein, which is bound to HDL and mediates the net transfer and exchange of phospholipids among different lipoproteins and participates in the transformation of larger HDL3 into smaller HDL2.	bind
56641	6	6859	6	10	NULL	0	NULL	statement 2			participate in					statement 5					NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_161_s_133	14592847	19 A candidate gene for  Hdlq19 is the gene ( Pltp; cM 93.0) coding for plasma phospholipid transfer protein, which is bound to HDL and mediates the net transfer and exchange of phospholipids among different lipoproteins and participates in the transformation of larger HDL3 into smaller HDL2.	bind
24277	1	6860	5	13	NULL	NULL	NULL	IRS-1	GP		bind					IR	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_988_s_160	12689920	19 Another possibility is that IRS-1 binds to IR with a higher affinity compared with IRS-2 or Shc 20,21  and therefore is a preferential substrate for IR. IRS-2 or Shc may become important only in the absence of IRS-1.	bind
24278	2	6860	5	13	NULL	NULL	NULL	IRS-2	GP		bind					IR	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_988_s_160	12689920	19 Another possibility is that IRS-1 binds to IR with a higher affinity compared with IRS-2 or Shc 20,21  and therefore is a preferential substrate for IR. IRS-2 or Shc may become important only in the absence of IRS-1.	bind
24279	3	6860	5	13	NULL	NULL	NULL	Shc	GP		bind					IR	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_988_s_160	12689920	19 Another possibility is that IRS-1 binds to IR with a higher affinity compared with IRS-2 or Shc 20,21  and therefore is a preferential substrate for IR. IRS-2 or Shc may become important only in the absence of IRS-1.	bind
24280	4	6860	5	13	NULL	NULL	NULL	statement 1	Process		has high affinity than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_988_s_160	12689920	19 Another possibility is that IRS-1 binds to IR with a higher affinity compared with IRS-2 or Shc 20,21  and therefore is a preferential substrate for IR. IRS-2 or Shc may become important only in the absence of IRS-1.	bind
24281	5	6860	5	13	NULL	NULL	NULL	statement 1	Process		has high affinity than					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_988_s_160	12689920	19 Another possibility is that IRS-1 binds to IR with a higher affinity compared with IRS-2 or Shc 20,21  and therefore is a preferential substrate for IR. IRS-2 or Shc may become important only in the absence of IRS-1.	bind
24282	6	6860	5	13	NULL	NULL	NULL	IRS-1	GP		is a substrate for		preferential			IR	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_988_s_160	12689920	19 Another possibility is that IRS-1 binds to IR with a higher affinity compared with IRS-2 or Shc 20,21  and therefore is a preferential substrate for IR. IRS-2 or Shc may become important only in the absence of IRS-1.	bind
24283	7	6860	5	13	NULL	NULL	NULL	IRS-2	GP		become important		may only			IRS-1	GP	in the absence of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_988_s_160	12689920	19 Another possibility is that IRS-1 binds to IR with a higher affinity compared with IRS-2 or Shc 20,21  and therefore is a preferential substrate for IR. IRS-2 or Shc may become important only in the absence of IRS-1.	bind
24284	8	6860	5	13	NULL	NULL	NULL	Shc	GP		become important		may only			IRS-1	GP	in the absence of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_988_s_160	12689920	19 Another possibility is that IRS-1 binds to IR with a higher affinity compared with IRS-2 or Shc 20,21  and therefore is a preferential substrate for IR. IRS-2 or Shc may become important only in the absence of IRS-1.	bind
20003	1	6860	6	10	NULL	0	NULL	IRS-1			bind					IR					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_988_s_160	12689920	19 Another possibility is that IRS-1 binds to IR with a higher affinity compared with IRS-2 or Shc 20,21  and therefore is a preferential substrate for IR. IRS-2 or Shc may become important only in the absence of IRS-1.	bind
20004	2	6860	6	NULL	NULL	0	NULL	IRS-2	NULL		bind	NULL				IR	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_988_s_160	12689920	19 Another possibility is that IRS-1 binds to IR with a higher affinity compared with IRS-2 or Shc 20,21  and therefore is a preferential substrate for IR. IRS-2 or Shc may become important only in the absence of IRS-1.	bind
20005	3	6860	6	NULL	NULL	0	NULL	Shc	NULL		bind	NULL				IR	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_988_s_160	12689920	19 Another possibility is that IRS-1 binds to IR with a higher affinity compared with IRS-2 or Shc 20,21  and therefore is a preferential substrate for IR. IRS-2 or Shc may become important only in the absence of IRS-1.	bind
56642	4	6860	6	10	NULL	0	NULL	statement 1			higher affinity than					statement 2					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_988_s_160	12689920	19 Another possibility is that IRS-1 binds to IR with a higher affinity compared with IRS-2 or Shc 20,21  and therefore is a preferential substrate for IR. IRS-2 or Shc may become important only in the absence of IRS-1.	bind
56643	5	6860	6	10	NULL	0	NULL	statement 1			higher affinity than					statement 3					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_988_s_160	12689920	19 Another possibility is that IRS-1 binds to IR with a higher affinity compared with IRS-2 or Shc 20,21  and therefore is a preferential substrate for IR. IRS-2 or Shc may become important only in the absence of IRS-1.	bind
56644	6	6860	6	10	NULL	0	NULL	 IRS-1			is substrate for		preferential			IR					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_988_s_160	12689920	19 Another possibility is that IRS-1 binds to IR with a higher affinity compared with IRS-2 or Shc 20,21  and therefore is a preferential substrate for IR. IRS-2 or Shc may become important only in the absence of IRS-1.	bind
56645	7	6860	6	10	NULL	0	NULL	IRS-2			become  important 		may			IRS-1		in the absence of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_988_s_160	12689920	19 Another possibility is that IRS-1 binds to IR with a higher affinity compared with IRS-2 or Shc 20,21  and therefore is a preferential substrate for IR. IRS-2 or Shc may become important only in the absence of IRS-1.	bind
56646	8	6860	6	10	NULL	0	NULL	Shc			become important 		may			IRS-1		in the absence of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_988_s_160	12689920	19 Another possibility is that IRS-1 binds to IR with a higher affinity compared with IRS-2 or Shc 20,21  and therefore is a preferential substrate for IR. IRS-2 or Shc may become important only in the absence of IRS-1.	bind
24285	1	6861	5	13	NULL	NULL	NULL	FKBP12.6	GP		bind					RyR	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_12_1213_s_47	16339492	19 Furthermore, FKBP12.6 binding to RyR is not affected during catecholamine stimulation that results in arrhythmias in a mouse model of catecholamine-induced ventricular tachycardia, 20,21  a genetic disorder of hypersensitive RyR Ca2+ release.	bind
24286	2	6861	5	13	NULL	NULL	NULL	statement 1	Process		is not affected during					catecholamine	Chemical	stimulation			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_12_1213_s_47	16339492	19 Furthermore, FKBP12.6 binding to RyR is not affected during catecholamine stimulation that results in arrhythmias in a mouse model of catecholamine-induced ventricular tachycardia, 20,21  a genetic disorder of hypersensitive RyR Ca2+ release.	bind
24287	3	6861	5	13	NULL	NULL	NULL	catecholamine	Chemical	stimulation with	results in					arrhythmias	MedicalFinding				NULL	 in a mouse model of catecholamine-induced ventricular tachycardia	NULL	NULL	NULL	NULL	gw70_circulationres_97_12_1213_s_47	16339492	19 Furthermore, FKBP12.6 binding to RyR is not affected during catecholamine stimulation that results in arrhythmias in a mouse model of catecholamine-induced ventricular tachycardia, 20,21  a genetic disorder of hypersensitive RyR Ca2+ release.	bind
56647	4	6861	5	13	NULL	NULL	NULL	ventricular tachycardia	MedicalFinding	catecholamine-induced	genetic disorder of					hypersensitive RyR Ca2+ release	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_12_1213_s_47	16339492	19 Furthermore, FKBP12.6 binding to RyR is not affected during catecholamine stimulation that results in arrhythmias in a mouse model of catecholamine-induced ventricular tachycardia, 20,21  a genetic disorder of hypersensitive RyR Ca2+ release.	bind
20006	1	6861	6	NULL	NULL	0	NULL	FKBP12.6	NULL		bind	NULL				RyR	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_12_1213_s_47	16339492	19 Furthermore, FKBP12.6 binding to RyR is not affected during catecholamine stimulation that results in arrhythmias in a mouse model of catecholamine-induced ventricular tachycardia, 20,21  a genetic disorder of hypersensitive RyR Ca2+ release.	bind
20007	2	6861	6	NULL	NULL	0	NULL	statement 1	NULL		is not affected during	NULL				catecholamine	NULL	stimulation by 			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_12_1213_s_47	16339492	19 Furthermore, FKBP12.6 binding to RyR is not affected during catecholamine stimulation that results in arrhythmias in a mouse model of catecholamine-induced ventricular tachycardia, 20,21  a genetic disorder of hypersensitive RyR Ca2+ release.	bind
20298	3	6861	6	NULL	NULL	0	NULL	catecholamine	NULL	stimulation by	results in	NULL				arrhythmias	NULL				NULL	mouse model	NULL	NULL	NULL	NULL	gw70_circulationres_97_12_1213_s_47	16339492	19 Furthermore, FKBP12.6 binding to RyR is not affected during catecholamine stimulation that results in arrhythmias in a mouse model of catecholamine-induced ventricular tachycardia, 20,21  a genetic disorder of hypersensitive RyR Ca2+ release.	bind
20299	4	6861	6	10	NULL	0	NULL	ventricular tachycardia		catecholamine-induced	is a genetic disorder of					hypersensitive RyR Ca2+ release					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_12_1213_s_47	16339492	19 Furthermore, FKBP12.6 binding to RyR is not affected during catecholamine stimulation that results in arrhythmias in a mouse model of catecholamine-induced ventricular tachycardia, 20,21  a genetic disorder of hypersensitive RyR Ca2+ release.	bind
24288	1	6862	5	13	NULL	NULL	NULL	hsp90	GP		bind					Akt	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_8_866_s_112	11988487	19 In cells, the binding of hsp90 to Akt prevents dephosphorylation of threonine 308 by reducing PP2A-mediated dephosphorylation.	bind
24289	2	6862	5	13	NULL	NULL	NULL	statement 1	Process		prevents							dephosphorylation of	threonine 308		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_8_866_s_112	11988487	19 In cells, the binding of hsp90 to Akt prevents dephosphorylation of threonine 308 by reducing PP2A-mediated dephosphorylation.	bind
24290	4	6862	5	13	NULL	NULL	NULL	statement 2	Process		occurs by reducing					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_8_866_s_112	11988487	19 In cells, the binding of hsp90 to Akt prevents dephosphorylation of threonine 308 by reducing PP2A-mediated dephosphorylation.	bind
44704	3	6862	5	13	NULL	NULL	NULL	PP2A	GP		mediates					dephosphorylation	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_8_866_s_112	11988487	19 In cells, the binding of hsp90 to Akt prevents dephosphorylation of threonine 308 by reducing PP2A-mediated dephosphorylation.	bind
20008	1	6862	6	NULL	NULL	0	NULL	hsp90	NULL		bind	NULL				Akt	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_8_866_s_112	11988487	19 In cells, the binding of hsp90 to Akt prevents dephosphorylation of threonine 308 by reducing PP2A-mediated dephosphorylation.	bind
20009	2	6862	6	10	NULL	0	NULL	statement 1			prevents							dephosphorylation of	threonine 308		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_8_866_s_112	11988487	19 In cells, the binding of hsp90 to Akt prevents dephosphorylation of threonine 308 by reducing PP2A-mediated dephosphorylation.	bind
20010	4	6862	6	10	NULL	0	NULL	statement 2			occurs by reducing					statement 3					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_8_866_s_112	11988487	19 In cells, the binding of hsp90 to Akt prevents dephosphorylation of threonine 308 by reducing PP2A-mediated dephosphorylation.	bind
56648	3	6862	6	10	NULL	0	NULL	PP2A			mediates					dephosphorylation					NULL		0	NULL	NULL	NULL	gw60_circulationres_90_8_866_s_112	11988487	19 In cells, the binding of hsp90 to Akt prevents dephosphorylation of threonine 308 by reducing PP2A-mediated dephosphorylation.	bind
24292	1	6863	5	13	NULL	NULL	NULL	ER transcript	NucleicAcid	short	is expressed in					mice	Organism				NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_1_120_s_171	12515753	19 In these mice, a short ER transcript is expressed that encodes an  N-terminal truncated, mutant ER that binds estrogen but possesses significantly reduced estrogen-dependent transcriptional activity compared with that of the wild-type ER, 20 resulting in the same functional domain changes as our findings with ERalpha-46 in human endothelial cells.	bind
24293	2	6863	5	13	NULL	NULL	NULL	statement 1	GP		encodes					ER	GP	truncated;;mutant 	N-terminal		NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_1_120_s_171	12515753	19 In these mice, a short ER transcript is expressed that encodes an  N-terminal truncated, mutant ER that binds estrogen but possesses significantly reduced estrogen-dependent transcriptional activity compared with that of the wild-type ER, 20 resulting in the same functional domain changes as our findings with ERalpha-46 in human endothelial cells.	bind
24294	3	6863	5	13	NULL	NULL	NULL	statement 2	GP		bind					estrogen	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_1_120_s_171	12515753	19 In these mice, a short ER transcript is expressed that encodes an  N-terminal truncated, mutant ER that binds estrogen but possesses significantly reduced estrogen-dependent transcriptional activity compared with that of the wild-type ER, 20 resulting in the same functional domain changes as our findings with ERalpha-46 in human endothelial cells.	bind
24295	4	6863	5	13	NULL	NULL	NULL	statement 2	GP		possesses		significantly			transcriptional activity	Process	estrogen-dependent			NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_1_120_s_171	12515753	19 In these mice, a short ER transcript is expressed that encodes an  N-terminal truncated, mutant ER that binds estrogen but possesses significantly reduced estrogen-dependent transcriptional activity compared with that of the wild-type ER, 20 resulting in the same functional domain changes as our findings with ERalpha-46 in human endothelial cells.	bind
24296	5	6863	5	13	NULL	NULL	NULL	ER	GP	wild-type	possesses					transcriptional activity 	Process	estrogen-dependent			NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_1_120_s_171	12515753	19 In these mice, a short ER transcript is expressed that encodes an  N-terminal truncated, mutant ER that binds estrogen but possesses significantly reduced estrogen-dependent transcriptional activity compared with that of the wild-type ER, 20 resulting in the same functional domain changes as our findings with ERalpha-46 in human endothelial cells.	bind
24297	6	6863	5	13	NULL	NULL	NULL	statement 4	Process		is reduced than					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_1_120_s_171	12515753	19 In these mice, a short ER transcript is expressed that encodes an  N-terminal truncated, mutant ER that binds estrogen but possesses significantly reduced estrogen-dependent transcriptional activity compared with that of the wild-type ER, 20 resulting in the same functional domain changes as our findings with ERalpha-46 in human endothelial cells.	bind
24298	7	6863	5	13	NULL	NULL	NULL	statement 6	Process		results in					functional domain changes	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_1_120_s_171	12515753	19 In these mice, a short ER transcript is expressed that encodes an  N-terminal truncated, mutant ER that binds estrogen but possesses significantly reduced estrogen-dependent transcriptional activity compared with that of the wild-type ER, 20 resulting in the same functional domain changes as our findings with ERalpha-46 in human endothelial cells.	bind
20041	2	6863	6	10	NULL	0	NULL	statement 1			bind					estrogen					NULL	mice	NULL	NULL	NULL	NULL	gw70_circulation_107_1_120_s_171	12515753	19 In these mice, a short ER transcript is expressed that encodes an  N-terminal truncated, mutant ER that binds estrogen but possesses significantly reduced estrogen-dependent transcriptional activity compared with that of the wild-type ER, 20 resulting in the same functional domain changes as our findings with ERalpha-46 in human endothelial cells.	bind
20042	3	6863	6	10	NULL	0	NULL	statement 2			possesses 					 transcriptional activity		estrogen-dependent			NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_1_120_s_171	12515753	19 In these mice, a short ER transcript is expressed that encodes an  N-terminal truncated, mutant ER that binds estrogen but possesses significantly reduced estrogen-dependent transcriptional activity compared with that of the wild-type ER, 20 resulting in the same functional domain changes as our findings with ERalpha-46 in human endothelial cells.	bind
20043	4	6863	6	10	NULL	0	NULL	ER		wild-type	possesses					transcriptional activity		estrogen-dependent			NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_1_120_s_171	12515753	19 In these mice, a short ER transcript is expressed that encodes an  N-terminal truncated, mutant ER that binds estrogen but possesses significantly reduced estrogen-dependent transcriptional activity compared with that of the wild-type ER, 20 resulting in the same functional domain changes as our findings with ERalpha-46 in human endothelial cells.	bind
20044	5	6863	6	10	NULL	0	NULL	statement 2			is reduced than		significantly			statement 3					NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_1_120_s_171	12515753	19 In these mice, a short ER transcript is expressed that encodes an  N-terminal truncated, mutant ER that binds estrogen but possesses significantly reduced estrogen-dependent transcriptional activity compared with that of the wild-type ER, 20 resulting in the same functional domain changes as our findings with ERalpha-46 in human endothelial cells.	bind
56649	1	6863	6	10	NULL	0	NULL	ER transcript		short	encode					ErbB2 receptor		mutant;;truncated	N-terminal		NULL	mice	NULL	NULL	NULL	NULL	gw70_circulation_107_1_120_s_171	12515753	19 In these mice, a short ER transcript is expressed that encodes an  N-terminal truncated, mutant ER that binds estrogen but possesses significantly reduced estrogen-dependent transcriptional activity compared with that of the wild-type ER, 20 resulting in the same functional domain changes as our findings with ERalpha-46 in human endothelial cells.	bind
56650	6	6863	6	10	NULL	0	NULL	statement 5			results in					functional domain changes					NULL		0	NULL	NULL	NULL	gw70_circulation_107_1_120_s_171	12515753	19 In these mice, a short ER transcript is expressed that encodes an  N-terminal truncated, mutant ER that binds estrogen but possesses significantly reduced estrogen-dependent transcriptional activity compared with that of the wild-type ER, 20 resulting in the same functional domain changes as our findings with ERalpha-46 in human endothelial cells.	bind
24299	1	6864	5	13	NULL	NULL	NULL	alpha-actinin	GP		bind					syndecan-4	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_7_674_s_243	16141413	19 Increased alpha-actinin binding to syndecan-4 may decrease cell motility, similar to the effect of overexpression of alpha-actinin.	bind
24300	2	6864	5	13	NULL	NULL	NULL	statement 1	Process	increased	decrease		may			cell motility	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_7_674_s_243	16141413	19 Increased alpha-actinin binding to syndecan-4 may decrease cell motility, similar to the effect of overexpression of alpha-actinin.	bind
24301	3	6864	5	13	NULL	NULL	NULL	alpha-actinin	GP	effect of overexpression of	is similar to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_7_674_s_243	16141413	19 Increased alpha-actinin binding to syndecan-4 may decrease cell motility, similar to the effect of overexpression of alpha-actinin.	bind
20011	1	6864	6	NULL	NULL	0	NULL	alpha-Actinin	NULL		bind	NULL				syndecan-4	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_7_674_s_243	16141413	19 Increased alpha-actinin binding to syndecan-4 may decrease cell motility, similar to the effect of overexpression of alpha-actinin.	bind
20045	2	6864	6	NULL	NULL	0	NULL	statement 1	NULL	increased	decrease	NULL	may			cell motility	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_7_674_s_243	16141413	19 Increased alpha-actinin binding to syndecan-4 may decrease cell motility, similar to the effect of overexpression of alpha-actinin.	bind
20046	3	6864	6	NULL	NULL	0	NULL	alpha-Actinin	NULL	overexpression of	decrease	NULL	may			cell motility	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_7_674_s_243	16141413	19 Increased alpha-actinin binding to syndecan-4 may decrease cell motility, similar to the effect of overexpression of alpha-actinin.	bind
24302	1	6866	5	13	NULL	NULL	NULL	Src	GP	activated	bind					PYK2	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_11_1790_s_33	12426206	19 The activated Src bound to PYK2 may phosphorylate PYK2 at Tyr579, Tyr580, and Tyr881, which promotes Grb2 (an adaptor protein) binding to PYK2 and enhances PYK2 kinase activity.	bind
24303	2	6866	5	13	NULL	NULL	NULL	statement 1	Process		phosphorylates		may			PYK2	GP		Tyr579		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_11_1790_s_33	12426206	19 The activated Src bound to PYK2 may phosphorylate PYK2 at Tyr579, Tyr580, and Tyr881, which promotes Grb2 (an adaptor protein) binding to PYK2 and enhances PYK2 kinase activity.	bind
24304	3	6866	5	13	NULL	NULL	NULL	statement 1	Process		phosphorylates		may			PYK2	GP		Tyr580		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_11_1790_s_33	12426206	19 The activated Src bound to PYK2 may phosphorylate PYK2 at Tyr579, Tyr580, and Tyr881, which promotes Grb2 (an adaptor protein) binding to PYK2 and enhances PYK2 kinase activity.	bind
24305	4	6866	5	13	NULL	NULL	NULL	statement 1	Process		phosphorylates		may			PYK2	GP		Tyr881		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_11_1790_s_33	12426206	19 The activated Src bound to PYK2 may phosphorylate PYK2 at Tyr579, Tyr580, and Tyr881, which promotes Grb2 (an adaptor protein) binding to PYK2 and enhances PYK2 kinase activity.	bind
24306	5	6866	5	13	NULL	NULL	NULL	Grb2	GP		is a type of					an adaptor protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_11_1790_s_33	12426206	19 The activated Src bound to PYK2 may phosphorylate PYK2 at Tyr579, Tyr580, and Tyr881, which promotes Grb2 (an adaptor protein) binding to PYK2 and enhances PYK2 kinase activity.	bind
24307	6	6866	5	13	NULL	NULL	NULL	Grb2	GP		bind					PYK2	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_11_1790_s_33	12426206	19 The activated Src bound to PYK2 may phosphorylate PYK2 at Tyr579, Tyr580, and Tyr881, which promotes Grb2 (an adaptor protein) binding to PYK2 and enhances PYK2 kinase activity.	bind
24308	7	6866	5	13	NULL	NULL	NULL	statement 2	Process		promote					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_11_1790_s_33	12426206	19 The activated Src bound to PYK2 may phosphorylate PYK2 at Tyr579, Tyr580, and Tyr881, which promotes Grb2 (an adaptor protein) binding to PYK2 and enhances PYK2 kinase activity.	bind
24309	8	6866	5	13	NULL	NULL	NULL	statement 3	Process		promote					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_11_1790_s_33	12426206	19 The activated Src bound to PYK2 may phosphorylate PYK2 at Tyr579, Tyr580, and Tyr881, which promotes Grb2 (an adaptor protein) binding to PYK2 and enhances PYK2 kinase activity.	bind
24310	9	6866	5	13	NULL	NULL	NULL	statement 4	Process		promote					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_11_1790_s_33	12426206	19 The activated Src bound to PYK2 may phosphorylate PYK2 at Tyr579, Tyr580, and Tyr881, which promotes Grb2 (an adaptor protein) binding to PYK2 and enhances PYK2 kinase activity.	bind
24311	10	6866	5	13	NULL	NULL	NULL	statement 2	Process		enhances					PYK2	GP	kinase activity of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_11_1790_s_33	12426206	19 The activated Src bound to PYK2 may phosphorylate PYK2 at Tyr579, Tyr580, and Tyr881, which promotes Grb2 (an adaptor protein) binding to PYK2 and enhances PYK2 kinase activity.	bind
24312	11	6866	5	13	NULL	NULL	NULL	statement 3	Process		enhances					PYK2	GP	kinase activity of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_11_1790_s_33	12426206	19 The activated Src bound to PYK2 may phosphorylate PYK2 at Tyr579, Tyr580, and Tyr881, which promotes Grb2 (an adaptor protein) binding to PYK2 and enhances PYK2 kinase activity.	bind
24313	12	6866	5	13	NULL	NULL	NULL	statement 4	Process		enhances					PYK2	GP	kinase activity of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_11_1790_s_33	12426206	19 The activated Src bound to PYK2 may phosphorylate PYK2 at Tyr579, Tyr580, and Tyr881, which promotes Grb2 (an adaptor protein) binding to PYK2 and enhances PYK2 kinase activity.	bind
20047	1	6866	6	NULL	NULL	0	NULL	Src	NULL	activated	bind	NULL				PYK2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_11_1790_s_33	12426206	19 The activated Src bound to PYK2 may phosphorylate PYK2 at Tyr579, Tyr580, and Tyr881, which promotes Grb2 (an adaptor protein) binding to PYK2 and enhances PYK2 kinase activity.	bind
20048	2	6866	6	NULL	NULL	0	NULL	Src	NULL	activated	phosphorylate	NULL	may			PYK2	NULL		Tyr579		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_11_1790_s_33	12426206	19 The activated Src bound to PYK2 may phosphorylate PYK2 at Tyr579, Tyr580, and Tyr881, which promotes Grb2 (an adaptor protein) binding to PYK2 and enhances PYK2 kinase activity.	bind
20049	3	6866	6	NULL	NULL	0	NULL	Src	NULL	activated	phosphorylate	NULL	may			PYK2	NULL		Tyr580		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_11_1790_s_33	12426206	19 The activated Src bound to PYK2 may phosphorylate PYK2 at Tyr579, Tyr580, and Tyr881, which promotes Grb2 (an adaptor protein) binding to PYK2 and enhances PYK2 kinase activity.	bind
20050	4	6866	6	NULL	NULL	0	NULL	Src	NULL	activated	phosphorylate	NULL	may			PYK2	NULL		Tyr881		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_11_1790_s_33	12426206	19 The activated Src bound to PYK2 may phosphorylate PYK2 at Tyr579, Tyr580, and Tyr881, which promotes Grb2 (an adaptor protein) binding to PYK2 and enhances PYK2 kinase activity.	bind
20051	5	6866	6	NULL	NULL	0	NULL	Grb2	NULL		bind	NULL				PYK2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_11_1790_s_33	12426206	19 The activated Src bound to PYK2 may phosphorylate PYK2 at Tyr579, Tyr580, and Tyr881, which promotes Grb2 (an adaptor protein) binding to PYK2 and enhances PYK2 kinase activity.	bind
20052	6	6866	6	10	NULL	0	NULL	Grb2	NULL		is a type of	NULL				adaptor protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_11_1790_s_33	12426206	19 The activated Src bound to PYK2 may phosphorylate PYK2 at Tyr579, Tyr580, and Tyr881, which promotes Grb2 (an adaptor protein) binding to PYK2 and enhances PYK2 kinase activity.	bind
20053	7	6866	6	NULL	NULL	0	NULL	statement 2	NULL		promotes	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_11_1790_s_33	12426206	19 The activated Src bound to PYK2 may phosphorylate PYK2 at Tyr579, Tyr580, and Tyr881, which promotes Grb2 (an adaptor protein) binding to PYK2 and enhances PYK2 kinase activity.	bind
20054	8	6866	6	NULL	NULL	0	NULL	statement 3	NULL		promotes	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_11_1790_s_33	12426206	19 The activated Src bound to PYK2 may phosphorylate PYK2 at Tyr579, Tyr580, and Tyr881, which promotes Grb2 (an adaptor protein) binding to PYK2 and enhances PYK2 kinase activity.	bind
20055	9	6866	6	NULL	NULL	0	NULL	statement 4	NULL		promotes	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_11_1790_s_33	12426206	19 The activated Src bound to PYK2 may phosphorylate PYK2 at Tyr579, Tyr580, and Tyr881, which promotes Grb2 (an adaptor protein) binding to PYK2 and enhances PYK2 kinase activity.	bind
20056	10	6866	6	NULL	NULL	0	NULL	statement 2	NULL		enhances	NULL				PYK2	NULL	kinase activity of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_11_1790_s_33	12426206	19 The activated Src bound to PYK2 may phosphorylate PYK2 at Tyr579, Tyr580, and Tyr881, which promotes Grb2 (an adaptor protein) binding to PYK2 and enhances PYK2 kinase activity.	bind
20057	11	6866	6	NULL	NULL	0	NULL	statement 3	NULL		enhances	NULL				PYK2	NULL	kinase activity of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_11_1790_s_33	12426206	19 The activated Src bound to PYK2 may phosphorylate PYK2 at Tyr579, Tyr580, and Tyr881, which promotes Grb2 (an adaptor protein) binding to PYK2 and enhances PYK2 kinase activity.	bind
20058	12	6866	6	NULL	NULL	0	NULL	statement 4	NULL		enhances	NULL				PYK2	NULL	kinase activity of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_11_1790_s_33	12426206	19 The activated Src bound to PYK2 may phosphorylate PYK2 at Tyr579, Tyr580, and Tyr881, which promotes Grb2 (an adaptor protein) binding to PYK2 and enhances PYK2 kinase activity.	bind
24314	1	6867	5	13	NULL	NULL	NULL	TIMP-3	GP		bind		high affinity			ECM 20	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_754_s_39	15681295	19 The high binding affinity of TIMP-3 to ECM 20 offers a further advantage, potentially retaining and concentrating TIMP-3 in the area around the stent struts and limiting its spread to the uninjured media.	bind
24315	2	6867	5	13	NULL	NULL	NULL	statement 1	Process		retains					TIMP-3	GP				NULL	in the area around stent struts	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_754_s_39	15681295	19 The high binding affinity of TIMP-3 to ECM 20 offers a further advantage, potentially retaining and concentrating TIMP-3 in the area around the stent struts and limiting its spread to the uninjured media.	bind
24316	3	6867	5	13	NULL	NULL	NULL	statement 1	Process		concentrates					TIMP-3	GP				NULL	in the area around stent struts	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_754_s_39	15681295	19 The high binding affinity of TIMP-3 to ECM 20 offers a further advantage, potentially retaining and concentrating TIMP-3 in the area around the stent struts and limiting its spread to the uninjured media.	bind
24317	4	6867	5	13	NULL	NULL	NULL	statement 1	Process		limits					TIMP-3	GP	spreading of			NULL	to uninjured media	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_754_s_39	15681295	19 The high binding affinity of TIMP-3 to ECM 20 offers a further advantage, potentially retaining and concentrating TIMP-3 in the area around the stent struts and limiting its spread to the uninjured media.	bind
20059	1	6867	6	NULL	NULL	0	NULL	TIMP-3	NULL		bind	NULL	high affinity			ECM 20	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_754_s_39	15681295	19 The high binding affinity of TIMP-3 to ECM 20 offers a further advantage, potentially retaining and concentrating TIMP-3 in the area around the stent struts and limiting its spread to the uninjured media.	bind
30290	2	6867	6	NULL	NULL	0	NULL	statement 1	NULL		retains	NULL				TIMP-3	NULL				NULL	in the area around stent struts	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_754_s_39	15681295	19 The high binding affinity of TIMP-3 to ECM 20 offers a further advantage, potentially retaining and concentrating TIMP-3 in the area around the stent struts and limiting its spread to the uninjured media.	bind
30291	3	6867	6	NULL	NULL	0	NULL	statement 1	NULL		concentrates	NULL				TIMP-3	NULL				NULL	in the area around stent struts	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_754_s_39	15681295	19 The high binding affinity of TIMP-3 to ECM 20 offers a further advantage, potentially retaining and concentrating TIMP-3 in the area around the stent struts and limiting its spread to the uninjured media.	bind
30292	4	6867	6	NULL	NULL	0	NULL	statement 1	NULL		limits	NULL				TIMP-3	NULL	spreading of			NULL	to uninjured media	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_754_s_39	15681295	19 The high binding affinity of TIMP-3 to ECM 20 offers a further advantage, potentially retaining and concentrating TIMP-3 in the area around the stent struts and limiting its spread to the uninjured media.	bind
24318	1	6868	5	13	NULL	NULL	NULL	CDR3	GP		bind					THP	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_5_1859_s_185	11337384	19, 20, 45  It is therefore interesting that CDR3 binds THP, although there are similarities in this region among many kappa and lambda light chains.	bind
20060	1	6868	6	NULL	NULL	0	NULL	CDR3	NULL		bind	NULL				THP	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_5_1859_s_185	11337384	19, 20, 45  It is therefore interesting that CDR3 binds THP, although there are similarities in this region among many kappa and lambda light chains.	bind
24319	1	6869	5	13	NULL	NULL	NULL	decorin	GP		regulates					collagen assembly	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_293	10934147	19, 36, 37  Besides regulating collagen assembly, decorin, biglycan, and fibromodulin can all bind TGF-beta1, -beta2, and -beta3, with fibromodulin exhibiting the greatest affinity for TGF-beta1, as well as the latent TGF-beta1 precursor.	bind
24320	2	6869	5	13	NULL	NULL	NULL	decorin	GP		bind					TGF-beta1	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_293	10934147	19, 36, 37  Besides regulating collagen assembly, decorin, biglycan, and fibromodulin can all bind TGF-beta1, -beta2, and -beta3, with fibromodulin exhibiting the greatest affinity for TGF-beta1, as well as the latent TGF-beta1 precursor.	bind
24321	3	6869	5	13	NULL	NULL	NULL	decorin	GP		bind					TGF-beta2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_293	10934147	19, 36, 37  Besides regulating collagen assembly, decorin, biglycan, and fibromodulin can all bind TGF-beta1, -beta2, and -beta3, with fibromodulin exhibiting the greatest affinity for TGF-beta1, as well as the latent TGF-beta1 precursor.	bind
24322	4	6869	5	13	NULL	NULL	NULL	decorin	GP		bind					TGF-beta3	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_293	10934147	19, 36, 37  Besides regulating collagen assembly, decorin, biglycan, and fibromodulin can all bind TGF-beta1, -beta2, and -beta3, with fibromodulin exhibiting the greatest affinity for TGF-beta1, as well as the latent TGF-beta1 precursor.	bind
24323	5	6869	5	13	NULL	NULL	NULL	biglycan	GP		regulates					collagen assembly	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_293	10934147	19, 36, 37  Besides regulating collagen assembly, decorin, biglycan, and fibromodulin can all bind TGF-beta1, -beta2, and -beta3, with fibromodulin exhibiting the greatest affinity for TGF-beta1, as well as the latent TGF-beta1 precursor.	bind
24324	6	6869	5	13	NULL	NULL	NULL	biglycan	GP		bind					TGF-beta1	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_293	10934147	19, 36, 37  Besides regulating collagen assembly, decorin, biglycan, and fibromodulin can all bind TGF-beta1, -beta2, and -beta3, with fibromodulin exhibiting the greatest affinity for TGF-beta1, as well as the latent TGF-beta1 precursor.	bind
24325	7	6869	5	13	NULL	NULL	NULL	biglycan	GP		bind					TGF-beta2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_293	10934147	19, 36, 37  Besides regulating collagen assembly, decorin, biglycan, and fibromodulin can all bind TGF-beta1, -beta2, and -beta3, with fibromodulin exhibiting the greatest affinity for TGF-beta1, as well as the latent TGF-beta1 precursor.	bind
24326	8	6869	5	13	NULL	NULL	NULL	biglycan	GP		bind					TGF-beta3	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_293	10934147	19, 36, 37  Besides regulating collagen assembly, decorin, biglycan, and fibromodulin can all bind TGF-beta1, -beta2, and -beta3, with fibromodulin exhibiting the greatest affinity for TGF-beta1, as well as the latent TGF-beta1 precursor.	bind
24327	9	6869	5	13	NULL	NULL	NULL	fibromodulin	GP		regulates					collagen assembly	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_293	10934147	19, 36, 37  Besides regulating collagen assembly, decorin, biglycan, and fibromodulin can all bind TGF-beta1, -beta2, and -beta3, with fibromodulin exhibiting the greatest affinity for TGF-beta1, as well as the latent TGF-beta1 precursor.	bind
24328	10	6869	5	13	NULL	NULL	NULL	fibromodulin	GP		bind					TGF-beta1	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_293	10934147	19, 36, 37  Besides regulating collagen assembly, decorin, biglycan, and fibromodulin can all bind TGF-beta1, -beta2, and -beta3, with fibromodulin exhibiting the greatest affinity for TGF-beta1, as well as the latent TGF-beta1 precursor.	bind
24329	11	6869	5	13	NULL	NULL	NULL	fibromodulin	GP		bind					TGF-beta2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_293	10934147	19, 36, 37  Besides regulating collagen assembly, decorin, biglycan, and fibromodulin can all bind TGF-beta1, -beta2, and -beta3, with fibromodulin exhibiting the greatest affinity for TGF-beta1, as well as the latent TGF-beta1 precursor.	bind
24330	12	6869	5	13	NULL	NULL	NULL	fibromodulin 	GP		bind					TGF-beta3	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_293	10934147	19, 36, 37  Besides regulating collagen assembly, decorin, biglycan, and fibromodulin can all bind TGF-beta1, -beta2, and -beta3, with fibromodulin exhibiting the greatest affinity for TGF-beta1, as well as the latent TGF-beta1 precursor.	bind
24331	13	6869	5	13	NULL	NULL	NULL	fibromodulin 	GP		affinity for		greatest			TGF-beta1 precursor	GP	latent			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_293	10934147	19, 36, 37  Besides regulating collagen assembly, decorin, biglycan, and fibromodulin can all bind TGF-beta1, -beta2, and -beta3, with fibromodulin exhibiting the greatest affinity for TGF-beta1, as well as the latent TGF-beta1 precursor.	bind
20061	1	6869	6	NULL	NULL	0	NULL	decorin	NULL		bind	NULL				TGF-beta1	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_293	10934147	19, 36, 37  Besides regulating collagen assembly, decorin, biglycan, and fibromodulin can all bind TGF-beta1, -beta2, and -beta3, with fibromodulin exhibiting the greatest affinity for TGF-beta1, as well as the latent TGF-beta1 precursor.	bind
20062	2	6869	6	NULL	NULL	0	NULL	decorin	NULL		bind	NULL				TGF-beta2	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_293	10934147	19, 36, 37  Besides regulating collagen assembly, decorin, biglycan, and fibromodulin can all bind TGF-beta1, -beta2, and -beta3, with fibromodulin exhibiting the greatest affinity for TGF-beta1, as well as the latent TGF-beta1 precursor.	bind
20063	3	6869	6	NULL	NULL	0	NULL	decorin	NULL		bind	NULL				TGF-beta3	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_293	10934147	19, 36, 37  Besides regulating collagen assembly, decorin, biglycan, and fibromodulin can all bind TGF-beta1, -beta2, and -beta3, with fibromodulin exhibiting the greatest affinity for TGF-beta1, as well as the latent TGF-beta1 precursor.	bind
20064	4	6869	6	NULL	NULL	0	NULL	biglycan	NULL		bind	NULL				TGF-beta1	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_293	10934147	19, 36, 37  Besides regulating collagen assembly, decorin, biglycan, and fibromodulin can all bind TGF-beta1, -beta2, and -beta3, with fibromodulin exhibiting the greatest affinity for TGF-beta1, as well as the latent TGF-beta1 precursor.	bind
20065	5	6869	6	NULL	NULL	0	NULL	biglycan	NULL		bind	NULL				TGF-beta2	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_293	10934147	19, 36, 37  Besides regulating collagen assembly, decorin, biglycan, and fibromodulin can all bind TGF-beta1, -beta2, and -beta3, with fibromodulin exhibiting the greatest affinity for TGF-beta1, as well as the latent TGF-beta1 precursor.	bind
20066	6	6869	6	NULL	NULL	0	NULL	biglycan	NULL		bind	NULL				TGF-beta3	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_293	10934147	19, 36, 37  Besides regulating collagen assembly, decorin, biglycan, and fibromodulin can all bind TGF-beta1, -beta2, and -beta3, with fibromodulin exhibiting the greatest affinity for TGF-beta1, as well as the latent TGF-beta1 precursor.	bind
20067	7	6869	6	NULL	NULL	0	NULL	fibromodulin	NULL		bind	NULL	high affinity			TGF-beta1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_293	10934147	19, 36, 37  Besides regulating collagen assembly, decorin, biglycan, and fibromodulin can all bind TGF-beta1, -beta2, and -beta3, with fibromodulin exhibiting the greatest affinity for TGF-beta1, as well as the latent TGF-beta1 precursor.	bind
20068	8	6869	6	NULL	NULL	0	NULL	fibromodulin	NULL		bind	NULL				TGF-beta2	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_293	10934147	19, 36, 37  Besides regulating collagen assembly, decorin, biglycan, and fibromodulin can all bind TGF-beta1, -beta2, and -beta3, with fibromodulin exhibiting the greatest affinity for TGF-beta1, as well as the latent TGF-beta1 precursor.	bind
20069	9	6869	6	NULL	NULL	0	NULL	fibromodulin	NULL		bind	NULL				TGF-beta3	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_293	10934147	19, 36, 37  Besides regulating collagen assembly, decorin, biglycan, and fibromodulin can all bind TGF-beta1, -beta2, and -beta3, with fibromodulin exhibiting the greatest affinity for TGF-beta1, as well as the latent TGF-beta1 precursor.	bind
30293	10	6869	6	NULL	NULL	0	NULL	decorin	NULL		regulate	NULL				collagen assembly	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_293	10934147	19, 36, 37  Besides regulating collagen assembly, decorin, biglycan, and fibromodulin can all bind TGF-beta1, -beta2, and -beta3, with fibromodulin exhibiting the greatest affinity for TGF-beta1, as well as the latent TGF-beta1 precursor.	bind
30294	11	6869	6	NULL	NULL	0	NULL	biglycan	NULL		regulate	NULL				collagen assembly	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_293	10934147	19, 36, 37  Besides regulating collagen assembly, decorin, biglycan, and fibromodulin can all bind TGF-beta1, -beta2, and -beta3, with fibromodulin exhibiting the greatest affinity for TGF-beta1, as well as the latent TGF-beta1 precursor.	bind
30295	12	6869	6	NULL	NULL	0	NULL	fibromodulin	NULL		regulate	NULL				collagen assembly	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_293	10934147	19, 36, 37  Besides regulating collagen assembly, decorin, biglycan, and fibromodulin can all bind TGF-beta1, -beta2, and -beta3, with fibromodulin exhibiting the greatest affinity for TGF-beta1, as well as the latent TGF-beta1 precursor.	bind
56651	13	6869	6	10	NULL	0	NULL	fibromodulin			affinity for		greatest 			TGF-beta1 precursor		latent			NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_2_423_s_293	10934147	19, 36, 37  Besides regulating collagen assembly, decorin, biglycan, and fibromodulin can all bind TGF-beta1, -beta2, and -beta3, with fibromodulin exhibiting the greatest affinity for TGF-beta1, as well as the latent TGF-beta1 precursor.	bind
24333	1	6870	5	13	NULL	NULL	NULL	HLA-G	GP		bind					ILT2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_71_s_182	11438456	19, [[ 20  This inhibition ]] is mediated by the binding of HLA-G to various inhibitory NKRs such as ILT2, ILT4, p49, and KIR2DL4.	bind
30355	2	6870	5	13	NULL	NULL	NULL	HLA-G	GP		bind					ILT4	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_71_s_182	11438456	19, [[ 20  This inhibition ]] is mediated by the binding of HLA-G to various inhibitory NKRs such as ILT2, ILT4, p49, and KIR2DL4.	bind
30356	3	6870	5	13	NULL	NULL	NULL	HLA-G	GP		bind					p49	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_71_s_182	11438456	19, [[ 20  This inhibition ]] is mediated by the binding of HLA-G to various inhibitory NKRs such as ILT2, ILT4, p49, and KIR2DL4.	bind
30357	4	6870	5	13	NULL	NULL	NULL	HLA-G	GP		bind					KIR2DL4	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_71_s_182	11438456	19, [[ 20  This inhibition ]] is mediated by the binding of HLA-G to various inhibitory NKRs such as ILT2, ILT4, p49, and KIR2DL4.	bind
56652	5	6870	5	13	NULL	NULL	NULL	ILT2	GP		is a type of					inhibitory NKR	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_71_s_182	11438456	19, [[ 20  This inhibition ]] is mediated by the binding of HLA-G to various inhibitory NKRs such as ILT2, ILT4, p49, and KIR2DL4.	bind
56653	6	6870	5	13	NULL	NULL	NULL	ILT4	GP		is a type of					inhibitory NKR	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_71_s_182	11438456	19, [[ 20  This inhibition ]] is mediated by the binding of HLA-G to various inhibitory NKRs such as ILT2, ILT4, p49, and KIR2DL4.	bind
56654	7	6870	5	13	NULL	NULL	NULL	p49	GP		is a type of					inhibitory NKR	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_71_s_182	11438456	19, [[ 20  This inhibition ]] is mediated by the binding of HLA-G to various inhibitory NKRs such as ILT2, ILT4, p49, and KIR2DL4.	bind
56655	8	6870	5	13	NULL	NULL	NULL	KIR2DL4	GP		is a type of					inhibitory NKR	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_71_s_182	11438456	19, [[ 20  This inhibition ]] is mediated by the binding of HLA-G to various inhibitory NKRs such as ILT2, ILT4, p49, and KIR2DL4.	bind
20119	1	6870	6	10	NULL	0	NULL	HLA-G			bind					ILT2					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_71_s_182	11438456	19, [[ 20  This inhibition ]] is mediated by the binding of HLA-G to various inhibitory NKRs such as ILT2, ILT4, p49, and KIR2DL4.	bind
20120	2	6870	6	10	NULL	0	NULL	HLA-G			bind					ILT4					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_71_s_182	11438456	19, [[ 20  This inhibition ]] is mediated by the binding of HLA-G to various inhibitory NKRs such as ILT2, ILT4, p49, and KIR2DL4.	bind
20121	3	6870	6	10	NULL	0	NULL	HLA-G			bind					p49 					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_71_s_182	11438456	19, [[ 20  This inhibition ]] is mediated by the binding of HLA-G to various inhibitory NKRs such as ILT2, ILT4, p49, and KIR2DL4.	bind
20122	4	6870	6	10	NULL	0	NULL	HLA-G			bind					KIR2DL4					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_71_s_182	11438456	19, [[ 20  This inhibition ]] is mediated by the binding of HLA-G to various inhibitory NKRs such as ILT2, ILT4, p49, and KIR2DL4.	bind
56656	5	6870	6	10	NULL	0	NULL	ILT2			is a type of					 inhibitory NKR					NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_1_71_s_182	11438456	19, [[ 20  This inhibition ]] is mediated by the binding of HLA-G to various inhibitory NKRs such as ILT2, ILT4, p49, and KIR2DL4.	bind
56657	6	6870	6	10	NULL	0	NULL	ILT4			is a type of					inhibitory NKR					NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_1_71_s_182	11438456	19, [[ 20  This inhibition ]] is mediated by the binding of HLA-G to various inhibitory NKRs such as ILT2, ILT4, p49, and KIR2DL4.	bind
56658	7	6870	6	10	NULL	0	NULL	p49			is a type of					inhibitory NKR					NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_1_71_s_182	11438456	19, [[ 20  This inhibition ]] is mediated by the binding of HLA-G to various inhibitory NKRs such as ILT2, ILT4, p49, and KIR2DL4.	bind
56659	8	6870	6	10	NULL	0	NULL	KIR2DL4			is a type of					inhibitory NKR					NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_1_71_s_182	11438456	19, [[ 20  This inhibition ]] is mediated by the binding of HLA-G to various inhibitory NKRs such as ILT2, ILT4, p49, and KIR2DL4.	bind
24338	1	6871	5	13	NULL	NULL	NULL	PAK	GP		is					p21-activated kinase	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1041_s_26	15016733	19,20  GIT proteins bind to p21-activated kinase (PAK), the downstream effector of Cdc42 and Rac, and a guanine nucleotide exchange factor termed PAK interacting exchange factor (PIX).	bind
24339	2	6871	5	13	NULL	NULL	NULL	GIT proteins	GP		bind					PAK	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1041_s_26	15016733	19,20  GIT proteins bind to p21-activated kinase (PAK), the downstream effector of Cdc42 and Rac, and a guanine nucleotide exchange factor termed PAK interacting exchange factor (PIX).	bind
24340	3	6871	5	13	NULL	NULL	NULL	PAK	GP		is a type of					downstream effector of Cdc42	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1041_s_26	15016733	19,20  GIT proteins bind to p21-activated kinase (PAK), the downstream effector of Cdc42 and Rac, and a guanine nucleotide exchange factor termed PAK interacting exchange factor (PIX).	bind
24341	4	6871	5	13	NULL	NULL	NULL	PAK	GP		is a type of					downstream effector of Rac	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1041_s_26	15016733	19,20  GIT proteins bind to p21-activated kinase (PAK), the downstream effector of Cdc42 and Rac, and a guanine nucleotide exchange factor termed PAK interacting exchange factor (PIX).	bind
24342	5	6871	5	13	NULL	NULL	NULL	PIX	GP		is					PAK interacting exchange factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1041_s_26	15016733	19,20  GIT proteins bind to p21-activated kinase (PAK), the downstream effector of Cdc42 and Rac, and a guanine nucleotide exchange factor termed PAK interacting exchange factor (PIX).	bind
24343	6	6871	5	13	NULL	NULL	NULL	GIT proteins	GP		bind					PIX	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1041_s_26	15016733	19,20  GIT proteins bind to p21-activated kinase (PAK), the downstream effector of Cdc42 and Rac, and a guanine nucleotide exchange factor termed PAK interacting exchange factor (PIX).	bind
44708	7	6871	5	13	NULL	NULL	NULL	PIX	GP		is a type of					guanine nucleotide exchange factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1041_s_26	15016733	19,20  GIT proteins bind to p21-activated kinase (PAK), the downstream effector of Cdc42 and Rac, and a guanine nucleotide exchange factor termed PAK interacting exchange factor (PIX).	bind
20123	1	6871	6	NULL	NULL	0	NULL	GIT protein	NULL		bind	NULL				PAK	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_8_1041_s_26	15016733	19,20  GIT proteins bind to p21-activated kinase (PAK), the downstream effector of Cdc42 and Rac, and a guanine nucleotide exchange factor termed PAK interacting exchange factor (PIX).	bind
20124	2	6871	6	NULL	NULL	0	NULL	PAK	NULL		is	NULL				p21-activated kinase	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_8_1041_s_26	15016733	19,20  GIT proteins bind to p21-activated kinase (PAK), the downstream effector of Cdc42 and Rac, and a guanine nucleotide exchange factor termed PAK interacting exchange factor (PIX).	bind
20125	3	6871	6	NULL	NULL	0	NULL	GIT protein	NULL		bind	NULL				PIX	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_8_1041_s_26	15016733	19,20  GIT proteins bind to p21-activated kinase (PAK), the downstream effector of Cdc42 and Rac, and a guanine nucleotide exchange factor termed PAK interacting exchange factor (PIX).	bind
20126	4	6871	6	NULL	NULL	0	NULL	PIX	NULL		is	NULL				PAK interacting exchange factor	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1041_s_26	15016733	19,20  GIT proteins bind to p21-activated kinase (PAK), the downstream effector of Cdc42 and Rac, and a guanine nucleotide exchange factor termed PAK interacting exchange factor (PIX).	bind
20127	5	6871	6	NULL	NULL	0	NULL	PIX	NULL		is a type of	NULL				guanine nucleotide exchange factor	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1041_s_26	15016733	19,20  GIT proteins bind to p21-activated kinase (PAK), the downstream effector of Cdc42 and Rac, and a guanine nucleotide exchange factor termed PAK interacting exchange factor (PIX).	bind
20128	6	6871	6	NULL	NULL	0	NULL	PAK	NULL		is a type of	NULL				downstream effector of Cdc42	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1041_s_26	15016733	19,20  GIT proteins bind to p21-activated kinase (PAK), the downstream effector of Cdc42 and Rac, and a guanine nucleotide exchange factor termed PAK interacting exchange factor (PIX).	bind
20129	7	6871	6	NULL	NULL	0	NULL	PAK	NULL		is a type of	NULL				downstream effector of Rac	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1041_s_26	15016733	19,20  GIT proteins bind to p21-activated kinase (PAK), the downstream effector of Cdc42 and Rac, and a guanine nucleotide exchange factor termed PAK interacting exchange factor (PIX).	bind
24344	1	6872	5	13	NULL	NULL	NULL	AT1	GP		bind					Ang II	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_9_965_s_38	15831814	19,20  Two main subtypes, AT1 and AT2 that bind mainly to Ang II and Ang III, have been cloned and extensively studied.	bind
24345	2	6872	5	13	NULL	NULL	NULL	AT2	GP		bind					Ang III	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_9_965_s_38	15831814	19,20  Two main subtypes, AT1 and AT2 that bind mainly to Ang II and Ang III, have been cloned and extensively studied.	bind
24346	3	6872	5	13	NULL	NULL	NULL	AT1	GP		bind					Ang III	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_9_965_s_38	15831814	19,20  Two main subtypes, AT1 and AT2 that bind mainly to Ang II and Ang III, have been cloned and extensively studied.	bind
24347	4	6872	5	13	NULL	NULL	NULL	AT2	GP		bind					Ang II	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_9_965_s_38	15831814	19,20  Two main subtypes, AT1 and AT2 that bind mainly to Ang II and Ang III, have been cloned and extensively studied.	bind
20130	1	6872	6	NULL	NULL	0	NULL	AT1	NULL		bind	NULL				Ang II	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_9_965_s_38	15831814	19,20  Two main subtypes, AT1 and AT2 that bind mainly to Ang II and Ang III, have been cloned and extensively studied.	bind
20131	2	6872	6	NULL	NULL	0	NULL	AT1	NULL		bind	NULL				Ang III	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_9_965_s_38	15831814	19,20  Two main subtypes, AT1 and AT2 that bind mainly to Ang II and Ang III, have been cloned and extensively studied.	bind
20132	3	6872	6	NULL	NULL	0	NULL	AT2	NULL		bind	NULL				Ang II	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_9_965_s_38	15831814	19,20  Two main subtypes, AT1 and AT2 that bind mainly to Ang II and Ang III, have been cloned and extensively studied.	bind
20133	4	6872	6	NULL	NULL	0	NULL	AT2	NULL		bind	NULL				Ang III	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_9_965_s_38	15831814	19,20  Two main subtypes, AT1 and AT2 that bind mainly to Ang II and Ang III, have been cloned and extensively studied.	bind
24589	1	6873	5	13	NULL	NULL	NULL	decorin	GP		bind					hydroxyapatite	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2391_s_35	15472131	19,23  Furthermore, decorin binds hydroxyapatite 24 and is localized to the newly developing fetal bone matrix at all stages of bone formation and within the matrix of resting nonarticular cartilage.	bind
24590	2	6873	5	13	NULL	NULL	NULL	statement 1	GP		is localized to					bone matrix	OrganismPart	newly developing fetal			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2391_s_35	15472131	19,23  Furthermore, decorin binds hydroxyapatite 24 and is localized to the newly developing fetal bone matrix at all stages of bone formation and within the matrix of resting nonarticular cartilage.	bind
24591	4	6873	5	13	NULL	NULL	NULL	statement 1	GP		is localized within					resting nonarticular cartilage	OrganismPart	matrix of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2391_s_35	15472131	19,23  Furthermore, decorin binds hydroxyapatite 24 and is localized to the newly developing fetal bone matrix at all stages of bone formation and within the matrix of resting nonarticular cartilage.	bind
30358	3	6873	5	13	NULL	NULL	NULL	statement 2	Process		occurs at					bone formation	Process	all stages of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2391_s_35	15472131	19,23  Furthermore, decorin binds hydroxyapatite 24 and is localized to the newly developing fetal bone matrix at all stages of bone formation and within the matrix of resting nonarticular cartilage.	bind
20134	1	6873	6	NULL	NULL	0	NULL	decorin	NULL		bind	NULL				hydroxyapatite	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2391_s_35	15472131	19,23  Furthermore, decorin binds hydroxyapatite 24 and is localized to the newly developing fetal bone matrix at all stages of bone formation and within the matrix of resting nonarticular cartilage.	bind
20135	2	6873	6	NULL	NULL	0	NULL	decorin	NULL		localized to	NULL				bone matrix	NULL	newly developing fetal			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2391_s_35	15472131	19,23  Furthermore, decorin binds hydroxyapatite 24 and is localized to the newly developing fetal bone matrix at all stages of bone formation and within the matrix of resting nonarticular cartilage.	bind
20262	3	6873	6	10	NULL	0	NULL	statement 2			occurs at					 bone formation		all stages of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2391_s_35	15472131	19,23  Furthermore, decorin binds hydroxyapatite 24 and is localized to the newly developing fetal bone matrix at all stages of bone formation and within the matrix of resting nonarticular cartilage.	bind
20263	4	6873	6	10	NULL	0	NULL	decorin			localized within					resting nonarticular cartilage		matrix of 			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2391_s_35	15472131	19,23  Furthermore, decorin binds hydroxyapatite 24 and is localized to the newly developing fetal bone matrix at all stages of bone formation and within the matrix of resting nonarticular cartilage.	bind
24592	1	6875	5	13	NULL	NULL	NULL	nerve growth factor receptor	GP		modulates					MAP kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_1931_s_1060	10688641	1992. ras mediates nerve growth factor receptor modulation of three signal-transducing protein kinases: MAP kinase, Raf-1, and RSK.	bind
24593	2	6875	5	13	NULL	NULL	NULL	nerve growth factor receptor	GP		modulates					Raf-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_1931_s_1060	10688641	1992. ras mediates nerve growth factor receptor modulation of three signal-transducing protein kinases: MAP kinase, Raf-1, and RSK.	bind
24594	3	6875	5	13	NULL	NULL	NULL	nerve growth factor receptor	GP		modulates					RSK	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_1931_s_1060	10688641	1992. ras mediates nerve growth factor receptor modulation of three signal-transducing protein kinases: MAP kinase, Raf-1, and RSK.	bind
24595	4	6875	5	13	NULL	NULL	NULL	ras	GP		mediates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_1931_s_1060	10688641	1992. ras mediates nerve growth factor receptor modulation of three signal-transducing protein kinases: MAP kinase, Raf-1, and RSK.	bind
24596	5	6875	5	13	NULL	NULL	NULL	ras	GP		mediates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_1931_s_1060	10688641	1992. ras mediates nerve growth factor receptor modulation of three signal-transducing protein kinases: MAP kinase, Raf-1, and RSK.	bind
24597	6	6875	5	13	NULL	NULL	NULL	ras	GP		mediates					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_1931_s_1060	10688641	1992. ras mediates nerve growth factor receptor modulation of three signal-transducing protein kinases: MAP kinase, Raf-1, and RSK.	bind
30359	7	6875	5	13	NULL	NULL	NULL	MAP kinase	GP		is a type of					signal-transducing protein kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_1931_s_1060	10688641	1992. ras mediates nerve growth factor receptor modulation of three signal-transducing protein kinases: MAP kinase, Raf-1, and RSK.	bind
30360	8	6875	5	13	NULL	NULL	NULL	Raf-1	GP		is a type of					signal-transducing protein kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_1931_s_1060	10688641	1992. ras mediates nerve growth factor receptor modulation of three signal-transducing protein kinases: MAP kinase, Raf-1, and RSK.	bind
30361	9	6875	5	13	NULL	NULL	NULL	RSK	GP		is a type of					signal-transducing protein kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_1931_s_1060	10688641	1992. ras mediates nerve growth factor receptor modulation of three signal-transducing protein kinases: MAP kinase, Raf-1, and RSK.	bind
20264	1	6875	6	NULL	NULL	0	NULL	nerve growth factor receptor	NULL		modulates	NULL				MAP kinase	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_6_1931_s_1060	10688641	1992. ras mediates nerve growth factor receptor modulation of three signal-transducing protein kinases: MAP kinase, Raf-1, and RSK.	bind
20265	2	6875	6	NULL	NULL	0	NULL	nerve growth factor receptor	NULL		modulates	NULL				Raf-1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_6_1931_s_1060	10688641	1992. ras mediates nerve growth factor receptor modulation of three signal-transducing protein kinases: MAP kinase, Raf-1, and RSK.	bind
20266	3	6875	6	NULL	NULL	0	NULL	nerve growth factor receptor	NULL		modulates	NULL				RSK	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_6_1931_s_1060	10688641	1992. ras mediates nerve growth factor receptor modulation of three signal-transducing protein kinases: MAP kinase, Raf-1, and RSK.	bind
20267	4	6875	6	NULL	NULL	0	NULL	ras	NULL		mediates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_6_1931_s_1060	10688641	1992. ras mediates nerve growth factor receptor modulation of three signal-transducing protein kinases: MAP kinase, Raf-1, and RSK.	bind
20268	5	6875	6	NULL	NULL	0	NULL	ras	NULL		mediates	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_6_1931_s_1060	10688641	1992. ras mediates nerve growth factor receptor modulation of three signal-transducing protein kinases: MAP kinase, Raf-1, and RSK.	bind
20269	6	6875	6	NULL	NULL	0	NULL	ras	NULL		mediates	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_6_1931_s_1060	10688641	1992. ras mediates nerve growth factor receptor modulation of three signal-transducing protein kinases: MAP kinase, Raf-1, and RSK.	bind
20270	7	6875	6	NULL	NULL	0	NULL	MAP kinase	NULL		is a type of	NULL				signal-transducing protein kinase	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_1931_s_1060	10688641	1992. ras mediates nerve growth factor receptor modulation of three signal-transducing protein kinases: MAP kinase, Raf-1, and RSK.	bind
20271	8	6875	6	NULL	NULL	0	NULL	Raf-1	NULL		is a type of	NULL				signal-transducing protein kinase	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_1931_s_1060	10688641	1992. ras mediates nerve growth factor receptor modulation of three signal-transducing protein kinases: MAP kinase, Raf-1, and RSK.	bind
20272	9	6875	6	NULL	NULL	0	NULL	RSK	NULL		is a type of	NULL				signal-transducing protein kinase	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_1931_s_1060	10688641	1992. ras mediates nerve growth factor receptor modulation of three signal-transducing protein kinases: MAP kinase, Raf-1, and RSK.	bind
24599	1	6878	5	13	NULL	NULL	NULL	OCI-5/glypican-3	GP	rat	bind					fibroblast growth factor-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_6_1407_s_493	9628896	1997. OCI-5/rat glypican-3 binds to fibroblast  growth factor-2 but not to insulin-like growth factor-2.	bind
24600	2	6878	5	13	NULL	NULL	NULL	OCI-5/glypican-3	GP	rat	does not bind					insulin-like growth factor-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_6_1407_s_493	9628896	1997. OCI-5/rat glypican-3 binds to fibroblast  growth factor-2 but not to insulin-like growth factor-2.	bind
20273	1	6878	6	NULL	NULL	0	NULL	OCI-5/glypican-3	NULL	Rat	bind	NULL				fibroblast growth factor-2	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_141_6_1407_s_493	9628896	1997. OCI-5/rat glypican-3 binds to fibroblast  growth factor-2 but not to insulin-like growth factor-2.	bind
20274	2	6878	6	NULL	NULL	0	NULL	OCI-5/glypican-3	NULL	rat	does not bind	NULL				insulin-like growth factor-2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_6_1407_s_493	9628896	1997. OCI-5/rat glypican-3 binds to fibroblast  growth factor-2 but not to insulin-like growth factor-2.	bind
24601	1	6879	5	13	NULL	NULL	NULL	arginine	AminoAcid		bind					ArgRS	GP	tRNA-free;;E. coli			NULL		NULL	NULL	NULL	NULL	gw60_febslett_547_1_197_s_110	12860413	19F NMR data at present illustrate that the 4-F-Trp162 resonance frequency is affected by the binding of arginine to tRNA-free  E. coli ArgRS, therefore suggesting that the local structure of Trp162 is involved in arginine binding.	bind
56660	2	6879	5	13	NULL	NULL	NULL				is involved in			Trp162		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_547_1_197_s_110	12860413	19F NMR data at present illustrate that the 4-F-Trp162 resonance frequency is affected by the binding of arginine to tRNA-free  E. coli ArgRS, therefore suggesting that the local structure of Trp162 is involved in arginine binding.	bind
20277	1	6879	6	10	NULL	0	NULL	arginine			bind					 ArgRS		tRNA-free;;E. coli			NULL		NULL	NULL	NULL	NULL	gw60_febslett_547_1_197_s_110	12860413	19F NMR data at present illustrate that the 4-F-Trp162 resonance frequency is affected by the binding of arginine to tRNA-free  E. coli ArgRS, therefore suggesting that the local structure of Trp162 is involved in arginine binding.	bind
20278	2	6879	6	NULL	NULL	0	NULL		NULL		is involved in	NULL		Trp162		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_547_1_197_s_110	12860413	19F NMR data at present illustrate that the 4-F-Trp162 resonance frequency is affected by the binding of arginine to tRNA-free  E. coli ArgRS, therefore suggesting that the local structure of Trp162 is involved in arginine binding.	bind
24605	1	6880	5	13	NULL	NULL	NULL	isoflurane	Chemical		bind		stereoselective			serum albumin	GP	bovine			NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_127_1_131_s_385	10369465	19F nuclear magnetic resonance investigation of stereoselective binding of isoflurane to bovine serum albumin.	bind
20279	1	6880	6	NULL	NULL	0	NULL	isoflurane	NULL		bind	NULL	stereoselectively			serum albumin	NULL	bovine			NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_127_1_131_s_385	10369465	19F nuclear magnetic resonance investigation of stereoselective binding of isoflurane to bovine serum albumin.	bind
24606	1	6882	5	13	NULL	NULL	NULL	1alpha,25(OH)2D3	Chemical		stimulates					MAP kinase	GP	phosphorylation of	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_4_2199_s_192	12417593	1alpha,25(OH)2D3 stimulation of MAP kinase tyrosine phosphorylation ( P) is suppressed by antibody inhibition of Raf-1.	bind
24607	3	6882	5	13	NULL	NULL	NULL	statement 2	Process		suppresses					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_4_2199_s_192	12417593	1alpha,25(OH)2D3 stimulation of MAP kinase tyrosine phosphorylation ( P) is suppressed by antibody inhibition of Raf-1.	bind
44829	2	6882	5	13	NULL	NULL	NULL	antibody	GP		inhibit					Raf-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_4_2199_s_192	12417593	1alpha,25(OH)2D3 stimulation of MAP kinase tyrosine phosphorylation ( P) is suppressed by antibody inhibition of Raf-1.	bind
44830	4	6882	5	13	NULL	NULL	NULL	P	Process		is					phosphorylation	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_4_2199_s_192	12417593	1alpha,25(OH)2D3 stimulation of MAP kinase tyrosine phosphorylation ( P) is suppressed by antibody inhibition of Raf-1.	bind
20280	1	6882	6	NULL	NULL	0	NULL	1alpha,25(OH)2D3	NULL		stimulates	NULL				MAP kinase	NULL	phosphorylation of	tyrosine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_4_2199_s_192	12417593	1alpha,25(OH)2D3 stimulation of MAP kinase tyrosine phosphorylation ( P) is suppressed by antibody inhibition of Raf-1.	bind
20281	2	6882	6	10	NULL	0	NULL	antibody	NULL		inhibits	NULL				Raf-1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_4_2199_s_192	12417593	1alpha,25(OH)2D3 stimulation of MAP kinase tyrosine phosphorylation ( P) is suppressed by antibody inhibition of Raf-1.	bind
20282	3	6882	6	NULL	NULL	0	NULL	P	NULL		is	NULL				phosphorylation	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_4_2199_s_192	12417593	1alpha,25(OH)2D3 stimulation of MAP kinase tyrosine phosphorylation ( P) is suppressed by antibody inhibition of Raf-1.	bind
44820	4	6882	6	10	NULL	0	NULL	statement 2	NULL		suppress	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_4_2199_s_192	12417593	1alpha,25(OH)2D3 stimulation of MAP kinase tyrosine phosphorylation ( P) is suppressed by antibody inhibition of Raf-1.	bind
24608	1	6884	5	13	NULL	NULL	NULL	1alpha,25(OH)2D3	Chemical		induces					Raf-1	GP	phosphorylation of	serine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_4_2199_s_118	12417593	1alpha,25(OH)2D3-induced serine phosphorylation ( P) of Raf-1 is suppressed by Ras inhibitor peptide.	bind
24609	2	6884	5	13	NULL	NULL	NULL	Ras inhibitor peptide	GP		suppresses					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_4_2199_s_118	12417593	1alpha,25(OH)2D3-induced serine phosphorylation ( P) of Raf-1 is suppressed by Ras inhibitor peptide.	bind
20283	1	6884	6	NULL	NULL	0	NULL	1alpha,25(OH)2D3	NULL		induce	NULL				Raf-1	NULL	phosphorylation of	Serine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_4_2199_s_118	12417593	1alpha,25(OH)2D3-induced serine phosphorylation ( P) of Raf-1 is suppressed by Ras inhibitor peptide.	bind
20284	2	6884	6	NULL	NULL	0	NULL	statement 1	NULL		is suppressed by	NULL				Ras inhibitor peptide	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_4_2199_s_118	12417593	1alpha,25(OH)2D3-induced serine phosphorylation ( P) of Raf-1 is suppressed by Ras inhibitor peptide.	bind
24610	1	6885	5	13	NULL	NULL	NULL	nucleotide	NucleicAcid		bind					Gialpha	GP	purified			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_26_27567_s_176	15096500	1b and GPR peptides derived from AGS4/G18.1b, PCP2, RapIGAPII,  and  C. elegans GPR-1/2 on nucleotide binding to purified Gialpha and Goalpha A, GTPgammaS binding to Gialpha (100 nM) was measured in the presence of increasing concentrations of GST, GST-AGS4/G18.	bind
24611	2	6885	5	13	NULL	NULL	NULL	GTPgammaS	Chemical		bind					Gialpha	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_26_27567_s_176	15096500	1b and GPR peptides derived from AGS4/G18.1b, PCP2, RapIGAPII,  and  C. elegans GPR-1/2 on nucleotide binding to purified Gialpha and Goalpha A, GTPgammaS binding to Gialpha (100 nM) was measured in the presence of increasing concentrations of GST, GST-AGS4/G18.	bind
30362	3	6885	5	13	NULL	NULL	NULL	nucleotide	NucleicAcid		bind					Goalpha A	GP	purified			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_26_27567_s_176	15096500	1b and GPR peptides derived from AGS4/G18.1b, PCP2, RapIGAPII,  and  C. elegans GPR-1/2 on nucleotide binding to purified Gialpha and Goalpha A, GTPgammaS binding to Gialpha (100 nM) was measured in the presence of increasing concentrations of GST, GST-AGS4/G18.	bind
20323	1	6885	6	NULL	NULL	0	NULL	nucleotide	NULL		bind	NULL				Gialpha	NULL	purified			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_26_27567_s_176	15096500	1b and GPR peptides derived from AGS4/G18.1b, PCP2, RapIGAPII,  and  C. elegans GPR-1/2 on nucleotide binding to purified Gialpha and Goalpha A, GTPgammaS binding to Gialpha (100 nM) was measured in the presence of increasing concentrations of GST, GST-AGS4/G18.	bind
20324	2	6885	6	NULL	NULL	0	NULL	nucleotide	NULL		bind	NULL				Goalpha A	NULL	purified			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_26_27567_s_176	15096500	1b and GPR peptides derived from AGS4/G18.1b, PCP2, RapIGAPII,  and  C. elegans GPR-1/2 on nucleotide binding to purified Gialpha and Goalpha A, GTPgammaS binding to Gialpha (100 nM) was measured in the presence of increasing concentrations of GST, GST-AGS4/G18.	bind
20325	3	6885	6	NULL	NULL	0	NULL	GTPgammaS	NULL		bind	NULL				Gialpha	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_26_27567_s_176	15096500	1b and GPR peptides derived from AGS4/G18.1b, PCP2, RapIGAPII,  and  C. elegans GPR-1/2 on nucleotide binding to purified Gialpha and Goalpha A, GTPgammaS binding to Gialpha (100 nM) was measured in the presence of increasing concentrations of GST, GST-AGS4/G18.	bind
24612	1	6887	5	13	NULL	NULL	NULL	1D6	GP		does not bind					peptide iB-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_1_380_s_12	9423886	1D6 did not bind peptide iB-1 but rather bound a second inhibitory epitope called iB-2.	bind
24613	2	6887	5	13	NULL	NULL	NULL	1D6	GP		bind					iB-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_1_380_s_12	9423886	1D6 did not bind peptide iB-1 but rather bound a second inhibitory epitope called iB-2.	bind
30363	3	6887	5	13	NULL	NULL	NULL	iB-2	GP		is a type of					inhibitory epitope	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_1_380_s_12	9423886	1D6 did not bind peptide iB-1 but rather bound a second inhibitory epitope called iB-2.	bind
20326	1	6887	6	10	NULL	0	NULL	1D6			does not bind					peptide iB-1					NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_1_380_s_12	9423886	1D6 did not bind peptide iB-1 but rather bound a second inhibitory epitope called iB-2.	bind
20327	2	6887	6	NULL	NULL	0	NULL	1D6	NULL		bind	NULL				iB2 	NULL				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_1_380_s_12	9423886	1D6 did not bind peptide iB-1 but rather bound a second inhibitory epitope called iB-2.	bind
30296	3	6887	6	NULL	NULL	0	NULL	iB2	NULL		is a type of	NULL				inhibitory epitope	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_1_380_s_12	9423886	1D6 did not bind peptide iB-1 but rather bound a second inhibitory epitope called iB-2.	bind
24614	1	6888	5	13	NULL	NULL	NULL	LDL receptor	GP		bind					apoE	GP	epitope of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_29	11557678	1D7 binds to the LDL receptor - binding epitope of apoE 15 and would therefore bind lipoproteins that had apoE in a metabolically active conformation.	bind
24615	2	6888	5	13	NULL	NULL	NULL	1D7	GP		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_29	11557678	1D7 binds to the LDL receptor - binding epitope of apoE 15 and would therefore bind lipoproteins that had apoE in a metabolically active conformation.	bind
24616	3	6888	5	13	NULL	NULL	NULL	lipoproteins	GP		contain					apoE	GP	metabolically active conformation			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_29	11557678	1D7 binds to the LDL receptor - binding epitope of apoE 15 and would therefore bind lipoproteins that had apoE in a metabolically active conformation.	bind
24617	4	6888	5	13	NULL	NULL	NULL	1D7	GP		bind					statement 3	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_29	11557678	1D7 binds to the LDL receptor - binding epitope of apoE 15 and would therefore bind lipoproteins that had apoE in a metabolically active conformation.	bind
24618	5	6888	5	13	NULL	NULL	NULL	statement 2	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_29	11557678	1D7 binds to the LDL receptor - binding epitope of apoE 15 and would therefore bind lipoproteins that had apoE in a metabolically active conformation.	bind
20328	1	6888	6	10	NULL	0	NULL	LDL receptor			bind					 apoE		epitope of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_29	11557678	1D7 binds to the LDL receptor - binding epitope of apoE 15 and would therefore bind lipoproteins that had apoE in a metabolically active conformation.	bind
20329	2	6888	6	NULL	NULL	0	NULL	1D7	NULL		bind	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_29	11557678	1D7 binds to the LDL receptor - binding epitope of apoE 15 and would therefore bind lipoproteins that had apoE in a metabolically active conformation.	bind
20731	3	6888	6	NULL	NULL	0	NULL	lipoproteins	NULL		contain	NULL				apoE	NULL	metabolically active conformation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_29	11557678	1D7 binds to the LDL receptor - binding epitope of apoE 15 and would therefore bind lipoproteins that had apoE in a metabolically active conformation.	bind
20732	4	6888	6	NULL	NULL	0	NULL	1D7	NULL		bind	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_29	11557678	1D7 binds to the LDL receptor - binding epitope of apoE 15 and would therefore bind lipoproteins that had apoE in a metabolically active conformation.	bind
56661	5	6888	6	10	NULL	0	NULL	statement 2			leads to					statement 4					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_29	11557678	1D7 binds to the LDL receptor - binding epitope of apoE 15 and would therefore bind lipoproteins that had apoE in a metabolically active conformation.	bind
24619	1	6890	5	13	NULL	NULL	NULL	VCAM-1	GP		bind					very late activation antibody-4	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_723_s_64	9598830	1G11, provided by Dr Dorian Haskard (Hammersmith Hospital, London) is an anti - VCAM-1 monoclonal antibody that blocks VCAM-1 binding to very late activation antibody-4.	bind
24620	2	6890	5	13	NULL	NULL	NULL	1G11	GP		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_723_s_64	9598830	1G11, provided by Dr Dorian Haskard (Hammersmith Hospital, London) is an anti - VCAM-1 monoclonal antibody that blocks VCAM-1 binding to very late activation antibody-4.	bind
30364	3	6890	5	13	NULL	NULL	NULL	1G11	GP		is a type of					anti - VCAM-1 monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_723_s_64	9598830	1G11, provided by Dr Dorian Haskard (Hammersmith Hospital, London) is an anti - VCAM-1 monoclonal antibody that blocks VCAM-1 binding to very late activation antibody-4.	bind
20330	1	6890	6	NULL	NULL	0	NULL	1G11	NULL		is a type of	NULL				anti - VCAM-1 monoclonal antibody 	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_723_s_64	9598830	1G11, provided by Dr Dorian Haskard (Hammersmith Hospital, London) is an anti - VCAM-1 monoclonal antibody that blocks VCAM-1 binding to very late activation antibody-4.	bind
20331	2	6890	6	NULL	NULL	0	NULL	VCAM-1	NULL		bind	NULL				very late activation antibody-4	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_723_s_64	9598830	1G11, provided by Dr Dorian Haskard (Hammersmith Hospital, London) is an anti - VCAM-1 monoclonal antibody that blocks VCAM-1 binding to very late activation antibody-4.	bind
20332	3	6890	6	NULL	NULL	0	NULL	1G11	NULL		blocks	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_723_s_64	9598830	1G11, provided by Dr Dorian Haskard (Hammersmith Hospital, London) is an anti - VCAM-1 monoclonal antibody that blocks VCAM-1 binding to very late activation antibody-4.	bind
24621	1	6891	5	13	NULL	NULL	NULL	SCN	Chemical		bind					HRP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_17_11049_s_35	9110998	1H and 15N NMR studies indicate that SCN  binds to HRP away from the distal histidine, near the heme methyl C1H3 and C18H3 with the  K d value of 158  plus-or-minus  19 mM and the binding is facilitated by protonation of an acid group with p K a 4.0 ( 38,  39).	bind
24622	2	6891	5	13	NULL	NULL	NULL	statement 1	Process		is facilitated by					acid group	Chemical	protonation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_17_11049_s_35	9110998	1H and 15N NMR studies indicate that SCN  binds to HRP away from the distal histidine, near the heme methyl C1H3 and C18H3 with the  K d value of 158  plus-or-minus  19 mM and the binding is facilitated by protonation of an acid group with p K a 4.0 ( 38,  39).	bind
30365	3	6891	5	13	NULL	NULL	NULL	statement 1	Process		occurs away from					HRP	GP	distal	histidine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_17_11049_s_35	9110998	1H and 15N NMR studies indicate that SCN  binds to HRP away from the distal histidine, near the heme methyl C1H3 and C18H3 with the  K d value of 158  plus-or-minus  19 mM and the binding is facilitated by protonation of an acid group with p K a 4.0 ( 38,  39).	bind
30366	4	6891	5	13	NULL	NULL	NULL	statement 1	Process		occurs near					HRP	GP		heme methyl  C1H3		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_17_11049_s_35	9110998	1H and 15N NMR studies indicate that SCN  binds to HRP away from the distal histidine, near the heme methyl C1H3 and C18H3 with the  K d value of 158  plus-or-minus  19 mM and the binding is facilitated by protonation of an acid group with p K a 4.0 ( 38,  39).	bind
30367	5	6891	5	13	NULL	NULL	NULL	statement 1	Process		occurs near					HRP	GP		heme methyl C18H3		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_17_11049_s_35	9110998	1H and 15N NMR studies indicate that SCN  binds to HRP away from the distal histidine, near the heme methyl C1H3 and C18H3 with the  K d value of 158  plus-or-minus  19 mM and the binding is facilitated by protonation of an acid group with p K a 4.0 ( 38,  39).	bind
20333	1	6891	6	NULL	NULL	0	NULL	SCN	NULL		bind	NULL				HRP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_17_11049_s_35	9110998	1H and 15N NMR studies indicate that SCN  binds to HRP away from the distal histidine, near the heme methyl C1H3 and C18H3 with the  K d value of 158  plus-or-minus  19 mM and the binding is facilitated by protonation of an acid group with p K a 4.0 ( 38,  39).	bind
20733	2	6891	6	10	NULL	0	NULL	statement 1			occurs away from					HRP		 distal	histidine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_17_11049_s_35	9110998	1H and 15N NMR studies indicate that SCN  binds to HRP away from the distal histidine, near the heme methyl C1H3 and C18H3 with the  K d value of 158  plus-or-minus  19 mM and the binding is facilitated by protonation of an acid group with p K a 4.0 ( 38,  39).	bind
20734	3	6891	6	NULL	NULL	0	NULL	statement 1	NULL		occurs near	NULL				HRP	NULL		heme methyl C1H3		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_17_11049_s_35	9110998	1H and 15N NMR studies indicate that SCN  binds to HRP away from the distal histidine, near the heme methyl C1H3 and C18H3 with the  K d value of 158  plus-or-minus  19 mM and the binding is facilitated by protonation of an acid group with p K a 4.0 ( 38,  39).	bind
20735	4	6891	6	NULL	NULL	0	NULL	statement 1	NULL		occurs near	NULL				HRP	NULL		heme methyl C18H3		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_17_11049_s_35	9110998	1H and 15N NMR studies indicate that SCN  binds to HRP away from the distal histidine, near the heme methyl C1H3 and C18H3 with the  K d value of 158  plus-or-minus  19 mM and the binding is facilitated by protonation of an acid group with p K a 4.0 ( 38,  39).	bind
56662	5	6891	6	10	NULL	0	NULL	statement 1			is facilitated by					acid group		protonation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_17_11049_s_35	9110998	1H and 15N NMR studies indicate that SCN  binds to HRP away from the distal histidine, near the heme methyl C1H3 and C18H3 with the  K d value of 158  plus-or-minus  19 mM and the binding is facilitated by protonation of an acid group with p K a 4.0 ( 38,  39).	bind
24623	1	6892	5	13	NULL	NULL	NULL	LMB	Chemical		bind					N-acetyl-L-cysteine methyl ester	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_16_9112_s_6	10430904	1H NMR analysis showed that LMB bound  N-acetyl-L-cysteine methyl ester through a Michael-type addition, consistent with the idea that LMB binds covalently via its alpha,beta-unsaturated delta-lactone to the sulfhydryl group of Cys-529.	bind
24624	2	6892	5	13	NULL	NULL	NULL	statement 1	Process		occurs through					Michael-type addition	ResearchActivity				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_16_9112_s_6	10430904	1H NMR analysis showed that LMB bound  N-acetyl-L-cysteine methyl ester through a Michael-type addition, consistent with the idea that LMB binds covalently via its alpha,beta-unsaturated delta-lactone to the sulfhydryl group of Cys-529.	bind
30368	3	6892	5	13	NULL	NULL	NULL	LMB	Chemical		bind		covalently	alpha,beta-unsaturated delta-lactone					sulfhydryl group of Cys-529		NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_16_9112_s_6	10430904	1H NMR analysis showed that LMB bound  N-acetyl-L-cysteine methyl ester through a Michael-type addition, consistent with the idea that LMB binds covalently via its alpha,beta-unsaturated delta-lactone to the sulfhydryl group of Cys-529.	bind
20357	1	6892	6	NULL	NULL	0	NULL	LMB	NULL		bind	NULL				N-acetyl-L-cysteine methyl ester	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_96_16_9112_s_6	10430904	1H NMR analysis showed that LMB bound  N-acetyl-L-cysteine methyl ester through a Michael-type addition, consistent with the idea that LMB binds covalently via its alpha,beta-unsaturated delta-lactone to the sulfhydryl group of Cys-529.	bind
20358	2	6892	6	NULL	NULL	0	NULL	LMB	NULL		bind	NULL	covalently	alpha,beta-unsaturated delta-lactone			NULL		sulfhydryl group of Cys-529		NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_16_9112_s_6	10430904	1H NMR analysis showed that LMB bound  N-acetyl-L-cysteine methyl ester through a Michael-type addition, consistent with the idea that LMB binds covalently via its alpha,beta-unsaturated delta-lactone to the sulfhydryl group of Cys-529.	bind
30297	3	6892	6	NULL	NULL	0	NULL	statement 1	NULL		occurs through	NULL				Michael-type addition	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_96_16_9112_s_6	10430904	1H NMR analysis showed that LMB bound  N-acetyl-L-cysteine methyl ester through a Michael-type addition, consistent with the idea that LMB binds covalently via its alpha,beta-unsaturated delta-lactone to the sulfhydryl group of Cys-529.	bind
24826	1	6893	5	13	NULL	NULL	NULL	Vpr1 - 40	GP		possesses					helical structure	GP		between residues 17 - 32		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_44_43188_s_6	12881523	1H NMR data indicate Vpr1 - 40 possesses helical structure between residues 17 - 32, and for the first time, this helix, which is bound by proline residues, was observed even in aqueous solution devoid of any detergent supplements.	bind
24827	2	6893	5	13	NULL	NULL	NULL	statement 1	GP		bind								proline residues		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_44_43188_s_6	12881523	1H NMR data indicate Vpr1 - 40 possesses helical structure between residues 17 - 32, and for the first time, this helix, which is bound by proline residues, was observed even in aqueous solution devoid of any detergent supplements.	bind
20361	1	6893	6	NULL	NULL	0	NULL	Vpr1-40	NULL		possesses	NULL				helical structure	NULL		between residues 17 - 32		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_44_43188_s_6	12881523	1H NMR data indicate Vpr1 - 40 possesses helical structure between residues 17 - 32, and for the first time, this helix, which is bound by proline residues, was observed even in aqueous solution devoid of any detergent supplements.	bind
20362	2	6893	6	10	NULL	0	NULL	statement 1			bind								proline residues		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_44_43188_s_6	12881523	1H NMR data indicate Vpr1 - 40 possesses helical structure between residues 17 - 32, and for the first time, this helix, which is bound by proline residues, was observed even in aqueous solution devoid of any detergent supplements.	bind
24828	1	6895	5	13	NULL	NULL	NULL	Pex14p	GP		bind								SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_5_1007_s_107	12453410	1H,15N correlation NMR spectra are shown for the uncomplexed (black) and the simultaneously Pex14p and Pex5p bound SH3 domain.	bind
24829	2	6895	5	13	NULL	NULL	NULL	Pex5p	GP		bind								SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_5_1007_s_107	12453410	1H,15N correlation NMR spectra are shown for the uncomplexed (black) and the simultaneously Pex14p and Pex5p bound SH3 domain.	bind
24830	3	6895	5	13	NULL	NULL	NULL	statement 1	Process		occurs simultaneously with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_5_1007_s_107	12453410	1H,15N correlation NMR spectra are shown for the uncomplexed (black) and the simultaneously Pex14p and Pex5p bound SH3 domain.	bind
20363	1	6895	6	NULL	NULL	0	NULL	Pex14p	NULL		bind	NULL					NULL		SH3 domain		NULL		0	NULL	NULL	NULL	gw60_molcell_10_5_1007_s_107	12453410	1H,15N correlation NMR spectra are shown for the uncomplexed (black) and the simultaneously Pex14p and Pex5p bound SH3 domain.	bind
20364	2	6895	6	NULL	NULL	0	NULL	Pex5p	NULL		bind	NULL					NULL		SH3 domain		NULL		0	NULL	NULL	NULL	gw60_molcell_10_5_1007_s_107	12453410	1H,15N correlation NMR spectra are shown for the uncomplexed (black) and the simultaneously Pex14p and Pex5p bound SH3 domain.	bind
30298	3	6895	6	NULL	NULL	0	NULL	statement 1	NULL		occurs simultaneously with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_10_5_1007_s_107	12453410	1H,15N correlation NMR spectra are shown for the uncomplexed (black) and the simultaneously Pex14p and Pex5p bound SH3 domain.	bind
24831	2	6896	5	13	NULL	NULL	NULL	[15N,2]cTnC	GP	Ca2+-saturated	bind					cTnI-AllP	GP		1-211		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_1_703_s_249	15507454	1H-15N correlation spectra of Ca2+-saturated [15N,2]cTnC bound to cTnI-WT-(1-211), cTnI-AllP-(1-211), or cTnI-PP-(1-211).	bind
24832	1	6896	5	13	NULL	NULL	NULL	[15N,2]cTnC	GP	Ca2+-saturated	bind					cTnI	GP	WT	1-211		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_1_703_s_249	15507454	1H-15N correlation spectra of Ca2+-saturated [15N,2]cTnC bound to cTnI-WT-(1-211), cTnI-AllP-(1-211), or cTnI-PP-(1-211).	bind
24833	3	6896	5	13	NULL	NULL	NULL	[15N,2]cTnC	GP	Ca2+-saturated	bind					cTnI-PP	GP		1-211		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_1_703_s_249	15507454	1H-15N correlation spectra of Ca2+-saturated [15N,2]cTnC bound to cTnI-WT-(1-211), cTnI-AllP-(1-211), or cTnI-PP-(1-211).	bind
20365	1	6896	6	10	NULL	0	NULL	[15N,2]cTnC		Ca2+ saturated	bind					cTnI		WT	1-211		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_1_703_s_249	15507454	1H-15N correlation spectra of Ca2+-saturated [15N,2]cTnC bound to cTnI-WT-(1-211), cTnI-AllP-(1-211), or cTnI-PP-(1-211).	bind
20366	2	6896	6	10	NULL	0	NULL	[15N,2]cTnC		Ca2+ saturated	bind					cTnI-AllP			1-211		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_1_703_s_249	15507454	1H-15N correlation spectra of Ca2+-saturated [15N,2]cTnC bound to cTnI-WT-(1-211), cTnI-AllP-(1-211), or cTnI-PP-(1-211).	bind
20367	3	6896	6	10	NULL	0	NULL	[15N,2]cTnC		Ca2+ saturated	bind					cTnI-PP			1-211		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_1_703_s_249	15507454	1H-15N correlation spectra of Ca2+-saturated [15N,2]cTnC bound to cTnI-WT-(1-211), cTnI-AllP-(1-211), or cTnI-PP-(1-211).	bind
24834	1	6897	5	13	NULL	NULL	NULL		GP		bind			C2A domain		syntaxin	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_18_1_133_s_56	9010211	1H-15N HSQC Cross-Peak Shifts Map the Region of the C2A Domain That Binds to Syntaxin	bind
20368	1	6897	6	NULL	NULL	0	NULL		NULL		bind	NULL		C2A domain		Syntaxin	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_18_1_133_s_56	9010211	1H-15N HSQC Cross-Peak Shifts Map the Region of the C2A Domain That Binds to Syntaxin	bind
24835	1	6898	5	13	NULL	NULL	NULL	complexin	GP		bind					SNARE Complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_33_3_397_s_50	11832227	1H-15N TROSY-HSQC Spectra Reveal the Region of Complexin that Binds to the SNARE Complex	bind
20369	1	6898	6	NULL	NULL	0	NULL	Complexin	NULL		bind	NULL				SNARE complex	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_33_3_397_s_50	11832227	1H-15N TROSY-HSQC Spectra Reveal the Region of Complexin that Binds to the SNARE Complex	bind
24836	1	6899	5	13	NULL	NULL	NULL	tau	GP		bind					tubulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_17_9503_s_196	10449722	1H-NMR studies suggest that the flexibility of tau can be changed, as shown by the fact that half of the methyl-containing residues of tau become immobilized on tau binding to tubulin ( 25).	bind
24837	2	6899	5	13	NULL	NULL	NULL	tau	GP		become			methyl residues		immobilized	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_17_9503_s_196	10449722	1H-NMR studies suggest that the flexibility of tau can be changed, as shown by the fact that half of the methyl-containing residues of tau become immobilized on tau binding to tubulin ( 25).	bind
24838	4	6899	5	13	NULL	NULL	NULL	statement 2	Process		suggests					tau	GP	change in flexibility of 			NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_17_9503_s_196	10449722	1H-NMR studies suggest that the flexibility of tau can be changed, as shown by the fact that half of the methyl-containing residues of tau become immobilized on tau binding to tubulin ( 25).	bind
30369	3	6899	5	13	NULL	NULL	NULL	statement 2	Process		occurs on					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_17_9503_s_196	10449722	1H-NMR studies suggest that the flexibility of tau can be changed, as shown by the fact that half of the methyl-containing residues of tau become immobilized on tau binding to tubulin ( 25).	bind
20370	1	6899	6	NULL	NULL	0	NULL	tau	NULL		bind	NULL				tubulin	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_96_17_9503_s_196	10449722	1H-NMR studies suggest that the flexibility of tau can be changed, as shown by the fact that half of the methyl-containing residues of tau become immobilized on tau binding to tubulin ( 25).	bind
20371	2	6899	6	NULL	NULL	0	NULL	tau	NULL		become	NULL		methyl residues		immobilized	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_96_17_9503_s_196	10449722	1H-NMR studies suggest that the flexibility of tau can be changed, as shown by the fact that half of the methyl-containing residues of tau become immobilized on tau binding to tubulin ( 25).	bind
20372	3	6899	6	NULL	NULL	0	NULL	statement 2	NULL		occurs during	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_96_17_9503_s_196	10449722	1H-NMR studies suggest that the flexibility of tau can be changed, as shown by the fact that half of the methyl-containing residues of tau become immobilized on tau binding to tubulin ( 25).	bind
56663	4	6899	6	10	NULL	0	NULL	statement 2			suggests					tau		change in flexibility of			NULL		0	NULL	NULL	NULL	gw60_pnas_96_17_9503_s_196	10449722	1H-NMR studies suggest that the flexibility of tau can be changed, as shown by the fact that half of the methyl-containing residues of tau become immobilized on tau binding to tubulin ( 25).	bind
20442	1	6900	6	NULL	NULL	0	NULL	S100B	NULL		bind	NULL				GST-alphaC28 pellet fraction	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_14_14382_s_198	14736868	1st lane, 2.5 muM S100B alone;  2nd lane, concentration of S100B bound in the 6 muM GST-alphaC28 pellet fraction;  3rd lane, nonspecific binding of S100B to glutathione-Sepharose resin alone;  4th lane, concentration of S100B bound in the 22 muM Affi-alphaC28 pellet fraction;  5th lane, nonspecific binding of S100B to Affi-Geltm resin alone.	bind
20444	2	6900	6	NULL	NULL	0	NULL	S100B	NULL		bind	NULL				Affi-alphaC28 pellet fraction	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_14_14382_s_198	14736868	1st lane, 2.5 muM S100B alone;  2nd lane, concentration of S100B bound in the 6 muM GST-alphaC28 pellet fraction;  3rd lane, nonspecific binding of S100B to glutathione-Sepharose resin alone;  4th lane, concentration of S100B bound in the 22 muM Affi-alphaC28 pellet fraction;  5th lane, nonspecific binding of S100B to Affi-Geltm resin alone.	bind
24840	1	6901	5	13	NULL	NULL	NULL	[CL3] RNA	NucleicAcid		bind					RNase III	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_9_2381_s_274	12711683	1[CL3] RNA binds RNase III in a manner distinct from that of a competent substrate.	bind
24841	2	6901	5	13	NULL	NULL	NULL	statement 1	Process		distinct from that of					competent substrate	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_9_2381_s_274	12711683	1[CL3] RNA binds RNase III in a manner distinct from that of a competent substrate.	bind
20447	1	6901	6	10	NULL	0	NULL	[CL3] RNA			bind					RNase III					NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_9_2381_s_274	12711683	1[CL3] RNA binds RNase III in a manner distinct from that of a competent substrate.	bind
56705	2	6901	6	10	NULL	0	NULL	statement 1			distinct from that of					competent substrate					NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_9_2381_s_274	12711683	1[CL3] RNA binds RNase III in a manner distinct from that of a competent substrate.	bind
24842	1	6902	5	13	NULL	NULL	NULL	[CL3] RNA	NucleicAcid		bind					RNase III	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_9_2381_s_290	12711683	1[CL3] RNA binds RNase III in the same manner as R1.1 RNA.	bind
24843	2	6902	5	13	NULL	NULL	NULL	R1.1 RNA	NucleicAcid		bind					RNase III	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_9_2381_s_290	12711683	1[CL3] RNA binds RNase III in the same manner as R1.1 RNA.	bind
24844	3	6902	5	13	NULL	NULL	NULL	statement 1	Process		same manner as					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_9_2381_s_290	12711683	1[CL3] RNA binds RNase III in the same manner as R1.1 RNA.	bind
20448	1	6902	6	NULL	NULL	0	NULL	RNA	NULL		bind	NULL				RNase III	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_9_2381_s_290	12711683	1[CL3] RNA binds RNase III in the same manner as R1.1 RNA.	bind
20449	2	6902	6	NULL	NULL	0	NULL	R1.1 RNA	NULL		bind	NULL				RNase III	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_9_2381_s_290	12711683	1[CL3] RNA binds RNase III in the same manner as R1.1 RNA.	bind
20450	3	6902	6	NULL	NULL	0	NULL	statement 1	NULL		occurs in the same manner as	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_9_2381_s_290	12711683	1[CL3] RNA binds RNase III in the same manner as R1.1 RNA.	bind
24848	1	6904	5	13	NULL	NULL	NULL	[CL3] RNA	NucleicAcid		is a variant of					 Class II R1.1 RNA	NucleicAcid	binding-competent;;cleavage-resistant			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_9_2381_s_238	12711683	1[CL3] RNA: a binding-competent, cleavage-resistant Class II R1.1 RNA variant   el shift assays revealed that none of the Class II R1.1 RNA variants are detectably bound by RNase III (data not shown), with one exception.	bind
24849	2	6904	5	13	NULL	NULL	NULL	Class II R1.1 RNA variants	NucleicAcid		does not bind					RNase III	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_9_2381_s_238	12711683	1[CL3] RNA: a binding-competent, cleavage-resistant Class II R1.1 RNA variant   el shift assays revealed that none of the Class II R1.1 RNA variants are detectably bound by RNase III (data not shown), with one exception.	bind
20456	1	6904	6	NULL	NULL	0	NULL	Class II R1.1 RNA variants	NULL		does not bind	NULL	detectably			RNase III	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_9_2381_s_238	12711683	1[CL3] RNA: a binding-competent, cleavage-resistant Class II R1.1 RNA variant   el shift assays revealed that none of the Class II R1.1 RNA variants are detectably bound by RNase III (data not shown), with one exception.	bind
30299	2	6904	6	NULL	NULL	0	NULL	[CL3] RNA	NULL		is a variant of	NULL				Class II R1.1 RNA	NULL	binding-competent;; cleavage-resistant			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_9_2381_s_238	12711683	1[CL3] RNA: a binding-competent, cleavage-resistant Class II R1.1 RNA variant   el shift assays revealed that none of the Class II R1.1 RNA variants are detectably bound by RNase III (data not shown), with one exception.	bind
24853	1	6906	5	13	NULL	NULL	NULL	 RNA	NucleicAcid		bind		efficiently			RNase III	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_25_13437_s_78	9391043	1[WC] RNA efficiently binds the RNase III mutant, the poorly cleaved substrates exhibit greatly weakened or undetectable binding (Fig.  3 A).	bind
20473	1	6906	6	NULL	NULL	0	NULL	RNA	NULL		bind	NULL	efficiently			RNase III	NULL	mutant			NULL		0	NULL	NULL	NULL	gw60_pnas_94_25_13437_s_78	9391043	1[WC] RNA efficiently binds the RNase III mutant, the poorly cleaved substrates exhibit greatly weakened or undetectable binding (Fig.  3 A).	bind
24854	1	6907	5	13	NULL	NULL	NULL	bacteriophage T5 5'' - 3' exonuclease	GP		bind		structure-specific			DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2772_s_257	11433022	2       Garforth,S.J. and Sayers,J.R. (1997) Structure-specific DNA binding by bacteriophage T5 5'' - 3' exonuclease.	bind
20474	1	6907	6	10	NULL	0	NULL	bacteriophage T5 5'' - 3' exonuclease	NULL		bind	NULL	Structure-specific			DNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2772_s_257	11433022	2       Garforth,S.J. and Sayers,J.R. (1997) Structure-specific DNA binding by bacteriophage T5 5'' - 3' exonuclease.	bind
24855	1	6909	5	13	NULL	NULL	NULL	telomerase	GP	yeast	bind			est1 subunit		tlc1 telomerase RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_11_2268_s_252	11376145	2       Zhou,J., Hidaka,K. and Futcher,B. (2000) The est1 subunit of yeast telomerase binds the tlc1 telomerase RNA.	bind
20475	1	6909	6	NULL	NULL	0	NULL	Telomerase	NULL	yeast	bind	NULL		est1 subunit		tlc1 telomerase RNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_11_2268_s_252	11376145	2       Zhou,J., Hidaka,K. and Futcher,B. (2000) The est1 subunit of yeast telomerase binds the tlc1 telomerase RNA.	bind
24856	1	6910	5	13	NULL	NULL	NULL	PAI-1	GP		bind					vitronectin	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_5112_s_343	9030577	2    In order to test for potential disruption of the PAI-1.vitronectin complex at the higher ionic strengths achieved in the quenching experiment, salt effects on the interaction were determined by comparing the binding of PAI-1 to immobilized vitronectin at 0.15 and 2 M NaCl.	bind
24857	2	6910	5	13	NULL	NULL	NULL	higher ionic strengths	QuantityOrMeasure		disrupts		potential			PAI-1.vitronectin complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_5112_s_343	9030577	2    In order to test for potential disruption of the PAI-1.vitronectin complex at the higher ionic strengths achieved in the quenching experiment, salt effects on the interaction were determined by comparing the binding of PAI-1 to immobilized vitronectin at 0.15 and 2 M NaCl.	bind
20477	1	6910	6	NULL	NULL	0	NULL	PAI	NULL		forms a complex with	NULL				vitronectin	NULL	immobilized			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_8_5112_s_343	9030577	2    In order to test for potential disruption of the PAI-1.vitronectin complex at the higher ionic strengths achieved in the quenching experiment, salt effects on the interaction were determined by comparing the binding of PAI-1 to immobilized vitronectin at 0.15 and 2 M NaCl.	bind
20478	2	6910	6	10	NULL	0	NULL	PAI-1.vitronectin complex 			is disrupted at					ionic strength		higher			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_5112_s_343	9030577	2    In order to test for potential disruption of the PAI-1.vitronectin complex at the higher ionic strengths achieved in the quenching experiment, salt effects on the interaction were determined by comparing the binding of PAI-1 to immobilized vitronectin at 0.15 and 2 M NaCl.	bind
24858	1	6915	5	13	NULL	NULL	NULL	iCpG DNA	NucleicAcid		bind					TLR9	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_25_22563_s_276	12695520	2  Although there is no formal demonstration that either CpG DNA or iCpG DNA  directly binds to TLR9, and the precise molecular mechanism by which iCpG DNA  blocks activity of CpG DNA has not been revealed, these previous studies  suggest that iCpG DNA may compete with CpG DNA for binding to TLR9.	bind
24859	2	6915	5	13	NULL	NULL	NULL	CpG DNA	NucleicAcid		bind					TLR9	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_25_22563_s_276	12695520	2  Although there is no formal demonstration that either CpG DNA or iCpG DNA  directly binds to TLR9, and the precise molecular mechanism by which iCpG DNA  blocks activity of CpG DNA has not been revealed, these previous studies  suggest that iCpG DNA may compete with CpG DNA for binding to TLR9.	bind
24860	3	6915	5	13	NULL	NULL	NULL	statement 1	Process		competes with		may			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_25_22563_s_276	12695520	2  Although there is no formal demonstration that either CpG DNA or iCpG DNA  directly binds to TLR9, and the precise molecular mechanism by which iCpG DNA  blocks activity of CpG DNA has not been revealed, these previous studies  suggest that iCpG DNA may compete with CpG DNA for binding to TLR9.	bind
24861	4	6915	5	13	NULL	NULL	NULL	iCpG DNA	NucleicAcid		blocks					CpG DNA	NucleicAcid	activity of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_25_22563_s_276	12695520	2  Although there is no formal demonstration that either CpG DNA or iCpG DNA  directly binds to TLR9, and the precise molecular mechanism by which iCpG DNA  blocks activity of CpG DNA has not been revealed, these previous studies  suggest that iCpG DNA may compete with CpG DNA for binding to TLR9.	bind
20480	1	6915	6	NULL	NULL	0	NULL	iCpG DNA	NULL		bind	NULL	directly			TLR9	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_25_22563_s_276	12695520	2  Although there is no formal demonstration that either CpG DNA or iCpG DNA  directly binds to TLR9, and the precise molecular mechanism by which iCpG DNA  blocks activity of CpG DNA has not been revealed, these previous studies  suggest that iCpG DNA may compete with CpG DNA for binding to TLR9.	bind
20481	2	6915	6	NULL	NULL	0	NULL	CpG DNA	NULL		bind	NULL	directly			TLR9	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_25_22563_s_276	12695520	2  Although there is no formal demonstration that either CpG DNA or iCpG DNA  directly binds to TLR9, and the precise molecular mechanism by which iCpG DNA  blocks activity of CpG DNA has not been revealed, these previous studies  suggest that iCpG DNA may compete with CpG DNA for binding to TLR9.	bind
20483	3	6915	6	NULL	NULL	0	NULL	statement 1	NULL		compete	NULL	may			statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_25_22563_s_276	12695520	2  Although there is no formal demonstration that either CpG DNA or iCpG DNA  directly binds to TLR9, and the precise molecular mechanism by which iCpG DNA  blocks activity of CpG DNA has not been revealed, these previous studies  suggest that iCpG DNA may compete with CpG DNA for binding to TLR9.	bind
20509	4	6915	6	NULL	NULL	0	NULL	iCpG DNA	NULL		blocks	NULL				CpG DNA	NULL	activity of 			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_25_22563_s_276	12695520	2  Although there is no formal demonstration that either CpG DNA or iCpG DNA  directly binds to TLR9, and the precise molecular mechanism by which iCpG DNA  blocks activity of CpG DNA has not been revealed, these previous studies  suggest that iCpG DNA may compete with CpG DNA for binding to TLR9.	bind
24862	1	6916	5	13	NULL	NULL	NULL	GP IIb/IIa	GP		interacts with					GP Ib/vWF	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_7_1124_s_20	9672073	2  GP IIb/IIa exists in an inactive state on resting platelets, but GP Ib/vWF interaction results in a conformational change within GP IIb/IIa, which then binds fibrinogen and vWF, resulting in platelet aggregation.	bind
24863	2	6916	5	13	NULL	NULL	NULL	statement 1	Process		results in					GP IIb/IIa	GP	conformational change within			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_7_1124_s_20	9672073	2  GP IIb/IIa exists in an inactive state on resting platelets, but GP Ib/vWF interaction results in a conformational change within GP IIb/IIa, which then binds fibrinogen and vWF, resulting in platelet aggregation.	bind
24864	3	6916	5	13	NULL	NULL	NULL	statement 2	GP		bind					fibrinogen	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_7_1124_s_20	9672073	2  GP IIb/IIa exists in an inactive state on resting platelets, but GP Ib/vWF interaction results in a conformational change within GP IIb/IIa, which then binds fibrinogen and vWF, resulting in platelet aggregation.	bind
24865	4	6916	5	13	NULL	NULL	NULL	statement 2	GP		bind					vWF	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_7_1124_s_20	9672073	2  GP IIb/IIa exists in an inactive state on resting platelets, but GP Ib/vWF interaction results in a conformational change within GP IIb/IIa, which then binds fibrinogen and vWF, resulting in platelet aggregation.	bind
24866	5	6916	5	13	NULL	NULL	NULL	statement 3	Process		results in					platelet	Cell	aggregation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_7_1124_s_20	9672073	2  GP IIb/IIa exists in an inactive state on resting platelets, but GP Ib/vWF interaction results in a conformational change within GP IIb/IIa, which then binds fibrinogen and vWF, resulting in platelet aggregation.	bind
24867	6	6916	5	13	NULL	NULL	NULL	statement 4	Process		results in					platelet	Cell	aggregation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_7_1124_s_20	9672073	2  GP IIb/IIa exists in an inactive state on resting platelets, but GP Ib/vWF interaction results in a conformational change within GP IIb/IIa, which then binds fibrinogen and vWF, resulting in platelet aggregation.	bind
20543	1	6916	6	10	NULL	0	NULL	GP IIb/IIa	NULL		interacts with	NULL				GP Ib/vWF	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_7_1124_s_20	9672073	2  GP IIb/IIa exists in an inactive state on resting platelets, but GP Ib/vWF interaction results in a conformational change within GP IIb/IIa, which then binds fibrinogen and vWF, resulting in platelet aggregation.	bind
20544	2	6916	6	10	NULL	0	NULL	statement 1	NULL		results in	NULL				GP IIb/IIa	NULL	conformational change within			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_7_1124_s_20	9672073	2  GP IIb/IIa exists in an inactive state on resting platelets, but GP Ib/vWF interaction results in a conformational change within GP IIb/IIa, which then binds fibrinogen and vWF, resulting in platelet aggregation.	bind
20545	3	6916	6	10	NULL	0	NULL	statement 2	NULL		bind	NULL				vWF	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_7_1124_s_20	9672073	2  GP IIb/IIa exists in an inactive state on resting platelets, but GP Ib/vWF interaction results in a conformational change within GP IIb/IIa, which then binds fibrinogen and vWF, resulting in platelet aggregation.	bind
20546	4	6916	6	10	NULL	0	NULL	statement 2	NULL		bind	NULL				fibrinogen	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_7_1124_s_20	9672073	2  GP IIb/IIa exists in an inactive state on resting platelets, but GP Ib/vWF interaction results in a conformational change within GP IIb/IIa, which then binds fibrinogen and vWF, resulting in platelet aggregation.	bind
20547	5	6916	6	10	NULL	0	NULL	statement 3	NULL		results in	NULL				platelet	NULL	aggregation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_7_1124_s_20	9672073	2  GP IIb/IIa exists in an inactive state on resting platelets, but GP Ib/vWF interaction results in a conformational change within GP IIb/IIa, which then binds fibrinogen and vWF, resulting in platelet aggregation.	bind
20548	6	6916	6	10	NULL	0	NULL	statement 4	NULL		results in	NULL				platelet	NULL	aggregation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_7_1124_s_20	9672073	2  GP IIb/IIa exists in an inactive state on resting platelets, but GP Ib/vWF interaction results in a conformational change within GP IIb/IIa, which then binds fibrinogen and vWF, resulting in platelet aggregation.	bind
24868	1	6917	5	13	NULL	NULL	NULL	Hsp47	GP		is					Heatshockprotein 47	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_11_1229_s_25	10725279	2  Heatshockprotein   47 (Hsp47) is a heat shock - inducible glycoprotein that binds nascent type I procollagen chains as they translocate into the endoplasmic reticulum.	bind
24869	2	6917	5	13	NULL	NULL	NULL	Hsp47	GP		bind					type I procollagen chains 	GP	nascent			NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_11_1229_s_25	10725279	2  Heatshockprotein   47 (Hsp47) is a heat shock - inducible glycoprotein that binds nascent type I procollagen chains as they translocate into the endoplasmic reticulum.	bind
24870	3	6917	5	13	NULL	NULL	NULL	type I procollagen chains 	GP	nascent	translocates into					endoplasmic reticulum	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_11_1229_s_25	10725279	2  Heatshockprotein   47 (Hsp47) is a heat shock - inducible glycoprotein that binds nascent type I procollagen chains as they translocate into the endoplasmic reticulum.	bind
24871	4	6917	5	13	NULL	NULL	NULL	statement 2	Process		occurs when					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_11_1229_s_25	10725279	2  Heatshockprotein   47 (Hsp47) is a heat shock - inducible glycoprotein that binds nascent type I procollagen chains as they translocate into the endoplasmic reticulum.	bind
30372	5	6917	5	13	NULL	NULL	NULL	Hsp47	GP		is a type of					heat shock-inducible glycoprotein	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_11_1229_s_25	10725279	2  Heatshockprotein   47 (Hsp47) is a heat shock - inducible glycoprotein that binds nascent type I procollagen chains as they translocate into the endoplasmic reticulum.	bind
20549	1	6917	6	10	NULL	0	NULL	Hsp47			is					Heatshockprotein 47					NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_11_1229_s_25	10725279	2  Heatshockprotein   47 (Hsp47) is a heat shock - inducible glycoprotein that binds nascent type I procollagen chains as they translocate into the endoplasmic reticulum.	bind
20550	2	6917	6	10	NULL	0	NULL	 type I procollagen chains		nascent	translocate into					endoplasmic reticulum					NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_11_1229_s_25	10725279	2  Heatshockprotein   47 (Hsp47) is a heat shock - inducible glycoprotein that binds nascent type I procollagen chains as they translocate into the endoplasmic reticulum.	bind
20551	3	6917	6	10	NULL	0	NULL	Hsp47			bind					 type I procollagen chains		nascent			NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_11_1229_s_25	10725279	2  Heatshockprotein   47 (Hsp47) is a heat shock - inducible glycoprotein that binds nascent type I procollagen chains as they translocate into the endoplasmic reticulum.	bind
20552	4	6917	6	NULL	NULL	0	NULL	Hsp47	NULL		is a type of	NULL				heat shock-inducible glycoprotein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_11_1229_s_25	10725279	2  Heatshockprotein   47 (Hsp47) is a heat shock - inducible glycoprotein that binds nascent type I procollagen chains as they translocate into the endoplasmic reticulum.	bind
56707	5	6917	6	10	NULL	0	NULL	statement 3			occurs upon					statement 2					NULL		0	NULL	NULL	NULL	gw60_circulation_101_11_1229_s_25	10725279	2  Heatshockprotein   47 (Hsp47) is a heat shock - inducible glycoprotein that binds nascent type I procollagen chains as they translocate into the endoplasmic reticulum.	bind
24872	1	6918	5	13	NULL	NULL	NULL	ANPR molecules	GP		occurs in					hh-dimer configuration	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_6115_s_252	14600147	2  In the ANP-bound complex structure, two ANPR molecules occur in the hh-dimer configuration, sandwiching one molecule of ANP.	bind
24873	2	6918	5	13	NULL	NULL	NULL	statement 1	GP		sandwich					 ANP	GP	one molecule of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_6115_s_252	14600147	2  In the ANP-bound complex structure, two ANPR molecules occur in the hh-dimer configuration, sandwiching one molecule of ANP.	bind
24874	3	6918	5	13	NULL	NULL	NULL	ANP-bound complex structure	GP		contains					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_6115_s_252	14600147	2  In the ANP-bound complex structure, two ANPR molecules occur in the hh-dimer configuration, sandwiching one molecule of ANP.	bind
56708	4	6918	5	13	NULL	NULL	NULL	statement 1	GP		occur in					ANP-bound complex structure	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_6115_s_252	14600147	2  In the ANP-bound complex structure, two ANPR molecules occur in the hh-dimer configuration, sandwiching one molecule of ANP.	bind
20553	1	6918	6	NULL	NULL	0	NULL	ANPR molecules	NULL		occur in	NULL				hh-dimer configuration	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_6115_s_252	14600147	2  In the ANP-bound complex structure, two ANPR molecules occur in the hh-dimer configuration, sandwiching one molecule of ANP.	bind
20554	2	6918	6	NULL	NULL	0	NULL	statement 1	NULL		occurs in	NULL				ANP-bound complex structure	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_6115_s_252	14600147	2  In the ANP-bound complex structure, two ANPR molecules occur in the hh-dimer configuration, sandwiching one molecule of ANP.	bind
20555	3	6918	6	10	NULL	0	NULL	ANPR molecules			sandwich					ANP		one molecule of 			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_6115_s_252	14600147	2  In the ANP-bound complex structure, two ANPR molecules occur in the hh-dimer configuration, sandwiching one molecule of ANP.	bind
20556	4	6918	6	10	NULL	0	NULL	ANP-bound complex structure			contains					statement 2					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_6115_s_252	14600147	2  In the ANP-bound complex structure, two ANPR molecules occur in the hh-dimer configuration, sandwiching one molecule of ANP.	bind
24875	1	6919	5	13	NULL	NULL	NULL	IP3	Chemical		bind					IP3 receptors	GP	specific			NULL	in smooth muscle cell	NULL	NULL	NULL	NULL	gw60_circulationres_84_5_536_s_15	10082475	2  IP3 binds to specific IP3 receptors in the smooth muscle cell, which produces a release of Ca2+ from the intracellular stores.	bind
24876	3	6919	5	13	NULL	NULL	NULL	statement 1	Process		produces					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_5_536_s_15	10082475	2  IP3 binds to specific IP3 receptors in the smooth muscle cell, which produces a release of Ca2+ from the intracellular stores.	bind
44744	2	6919	5	13	NULL	NULL	NULL	Ca2+	Chemical		released from					intracellular stores	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_5_536_s_15	10082475	2  IP3 binds to specific IP3 receptors in the smooth muscle cell, which produces a release of Ca2+ from the intracellular stores.	bind
20557	1	6919	6	NULL	NULL	0	NULL	IP3	NULL		bind	NULL				IP3 receptors	NULL	specific			NULL	smooth muscle cell	NULL	NULL	NULL	NULL	gw60_circulationres_84_5_536_s_15	10082475	2  IP3 binds to specific IP3 receptors in the smooth muscle cell, which produces a release of Ca2+ from the intracellular stores.	bind
20558	2	6919	6	NULL	NULL	0	NULL	Ca2+	NULL		released from	NULL				intracellular stores	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_5_536_s_15	10082475	2  IP3 binds to specific IP3 receptors in the smooth muscle cell, which produces a release of Ca2+ from the intracellular stores.	bind
20559	3	6919	6	NULL	NULL	0	NULL	statement 1	NULL		produces	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_5_536_s_15	10082475	2  IP3 binds to specific IP3 receptors in the smooth muscle cell, which produces a release of Ca2+ from the intracellular stores.	bind
24877	1	6920	5	13	NULL	NULL	NULL	DCoH/PCD molecules	GP		bind					HNF1 dimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_6_2021_s_13	11395380	2  It has been shown that two DCoH/PCD molecules bind to a HNF1 dimer forming a transcriptionally active heterotetrameric complex.	bind
24878	2	6920	5	13	NULL	NULL	NULL	statement 1	GP		forms					heterotetrameric complex	GP	transcriptionally active			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_6_2021_s_13	11395380	2  It has been shown that two DCoH/PCD molecules bind to a HNF1 dimer forming a transcriptionally active heterotetrameric complex.	bind
20560	1	6920	6	NULL	NULL	0	NULL	DcoH/PCD molecules	NULL		bind	NULL				HNF1 dimer	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_6_2021_s_13	11395380	2  It has been shown that two DCoH/PCD molecules bind to a HNF1 dimer forming a transcriptionally active heterotetrameric complex.	bind
20561	2	6920	6	NULL	NULL	0	NULL	statement 1	NULL		forms a 	NULL				heterotetrameric complex	NULL	transcriptionally active 			NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_6_2021_s_13	11395380	2  It has been shown that two DCoH/PCD molecules bind to a HNF1 dimer forming a transcriptionally active heterotetrameric complex.	bind
24879	1	6921	5	13	NULL	NULL	NULL	fibrinogen	GP		bind					GP IIb/IIa receptor	GP	activated form 			NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_9_1013_s_19	10704169	2  Platelet aggregation is mediated through the binding of fibrinogen or von Willebrand factor (vWF) to the activated form of the platelet glycoprotein (GP) IIb/IIa (integrin alphaIIbbeta3) receptor.	bind
24880	2	6921	5	13	NULL	NULL	NULL	GP	GP		is					platelet glycoprotein	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_9_1013_s_19	10704169	2  Platelet aggregation is mediated through the binding of fibrinogen or von Willebrand factor (vWF) to the activated form of the platelet glycoprotein (GP) IIb/IIa (integrin alphaIIbbeta3) receptor.	bind
24960	3	6921	5	13	NULL	NULL	NULL	platelet	Process	aggregation of	is mediated through					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_9_1013_s_19	10704169	2  Platelet aggregation is mediated through the binding of fibrinogen or von Willebrand factor (vWF) to the activated form of the platelet glycoprotein (GP) IIb/IIa (integrin alphaIIbbeta3) receptor.	bind
24961	4	6921	5	13	NULL	NULL	NULL	vWF	GP		is					von Willebrand factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_9_1013_s_19	10704169	2  Platelet aggregation is mediated through the binding of fibrinogen or von Willebrand factor (vWF) to the activated form of the platelet glycoprotein (GP) IIb/IIa (integrin alphaIIbbeta3) receptor.	bind
24963	5	6921	5	13	NULL	NULL	NULL	vWF	GP		bind					GP IIb/IIa receptor	GP	activated form			NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_9_1013_s_19	10704169	2  Platelet aggregation is mediated through the binding of fibrinogen or von Willebrand factor (vWF) to the activated form of the platelet glycoprotein (GP) IIb/IIa (integrin alphaIIbbeta3) receptor.	bind
24964	6	6921	5	13	NULL	NULL	NULL	platelet	Process	aggregation of	is mediated through					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_9_1013_s_19	10704169	2  Platelet aggregation is mediated through the binding of fibrinogen or von Willebrand factor (vWF) to the activated form of the platelet glycoprotein (GP) IIb/IIa (integrin alphaIIbbeta3) receptor.	bind
24965	7	6921	5	13	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_9_1013_s_19	10704169	2  Platelet aggregation is mediated through the binding of fibrinogen or von Willebrand factor (vWF) to the activated form of the platelet glycoprotein (GP) IIb/IIa (integrin alphaIIbbeta3) receptor.	bind
56713	8	6921	5	13	NULL	NULL	NULL	IIb/IIa	GP		is					integrin alphaIIbbeta3	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_9_1013_s_19	10704169	2  Platelet aggregation is mediated through the binding of fibrinogen or von Willebrand factor (vWF) to the activated form of the platelet glycoprotein (GP) IIb/IIa (integrin alphaIIbbeta3) receptor.	bind
20562	1	6921	6	NULL	NULL	0	NULL	vWF	NULL		is	NULL				von Willebrand factor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_101_9_1013_s_19	10704169	2  Platelet aggregation is mediated through the binding of fibrinogen or von Willebrand factor (vWF) to the activated form of the platelet glycoprotein (GP) IIb/IIa (integrin alphaIIbbeta3) receptor.	bind
20563	2	6921	6	NULL	NULL	0	NULL	fibrinogen	NULL		bind	NULL				GP IIb/IIa receptor	NULL	activated form			NULL		0	NULL	NULL	NULL	gw60_circulation_101_9_1013_s_19	10704169	2  Platelet aggregation is mediated through the binding of fibrinogen or von Willebrand factor (vWF) to the activated form of the platelet glycoprotein (GP) IIb/IIa (integrin alphaIIbbeta3) receptor.	bind
20564	3	6921	6	NULL	NULL	0	NULL	vWF	NULL		bind	NULL				GP IIb/IIa receptor	NULL	activated form			NULL		0	NULL	NULL	NULL	gw60_circulation_101_9_1013_s_19	10704169	2  Platelet aggregation is mediated through the binding of fibrinogen or von Willebrand factor (vWF) to the activated form of the platelet glycoprotein (GP) IIb/IIa (integrin alphaIIbbeta3) receptor.	bind
20566	8	6921	6	10	NULL	0	NULL	GP			is					platelet glycoprotein					NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_9_1013_s_19	10704169	2  Platelet aggregation is mediated through the binding of fibrinogen or von Willebrand factor (vWF) to the activated form of the platelet glycoprotein (GP) IIb/IIa (integrin alphaIIbbeta3) receptor.	bind
20567	6	6921	6	10	NULL	0	NULL	 IIb/IIa			is					integrin alphaIIbbeta3					NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_9_1013_s_19	10704169	2  Platelet aggregation is mediated through the binding of fibrinogen or von Willebrand factor (vWF) to the activated form of the platelet glycoprotein (GP) IIb/IIa (integrin alphaIIbbeta3) receptor.	bind
56709	4	6921	6	10	NULL	0	NULL	platelet		aggregation of	is mediated through					statement 2					NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_9_1013_s_19	10704169	2  Platelet aggregation is mediated through the binding of fibrinogen or von Willebrand factor (vWF) to the activated form of the platelet glycoprotein (GP) IIb/IIa (integrin alphaIIbbeta3) receptor.	bind
56710	5	6921	6	10	NULL	0	NULL	platelet		aggregation of	is mediated through					statement 3					NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_9_1013_s_19	10704169	2  Platelet aggregation is mediated through the binding of fibrinogen or von Willebrand factor (vWF) to the activated form of the platelet glycoprotein (GP) IIb/IIa (integrin alphaIIbbeta3) receptor.	bind
56712	7	6921	6	10	NULL	0	NULL	statement 4			is an alternative to					statement 5					NULL		0	NULL	NULL	NULL	gw60_circulation_101_9_1013_s_19	10704169	2  Platelet aggregation is mediated through the binding of fibrinogen or von Willebrand factor (vWF) to the activated form of the platelet glycoprotein (GP) IIb/IIa (integrin alphaIIbbeta3) receptor.	bind
24966	1	6922	5	13	NULL	NULL	NULL				overlaps				cryptic element	PDGF-B	GP			Sp1 site in promoter	NULL	in cells exposed to PMA	NULL	NULL	NULL	NULL	gw60_circulationres_81_4_457_s_29	9314825	2  Similar strategies later revealed that Egr-1 binds to a cryptic element overlapping the Sp1 site in the PDGF-B promoter in cells exposed to PMA. 9	bind
24967	2	6922	5	13	NULL	NULL	NULL	Egr-1	GP		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_81_4_457_s_29	9314825	2  Similar strategies later revealed that Egr-1 binds to a cryptic element overlapping the Sp1 site in the PDGF-B promoter in cells exposed to PMA. 9	bind
20568	2	6922	6	10	NULL	0	NULL	Egr-1			bind					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_81_4_457_s_29	9314825	2  Similar strategies later revealed that Egr-1 binds to a cryptic element overlapping the Sp1 site in the PDGF-B promoter in cells exposed to PMA. 9	bind
56714	1	6922	6	10	NULL	0	NULL				overlaps				cryptic element	PDGF-B				Sp1 site in promoter	NULL	cells exposed to PMA	0	NULL	NULL	NULL	gw60_circulationres_81_4_457_s_29	9314825	2  Similar strategies later revealed that Egr-1 binds to a cryptic element overlapping the Sp1 site in the PDGF-B promoter in cells exposed to PMA. 9	bind
24968	2	6923	5	13	NULL	NULL	NULL	hydrophobic contact	Process		stabilize			Phe96A-Phe96B		statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_6115_s_277	14600147	2  The hydrophobic contact Phe96A-Phe96B remains and apparently contributes to stabilizing the ANP-bound activated complex.	bind
44709	1	6923	5	13	NULL	NULL	NULL	ANP	GP		bind					activated complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_6115_s_277	14600147	2  The hydrophobic contact Phe96A-Phe96B remains and apparently contributes to stabilizing the ANP-bound activated complex.	bind
20590	2	6923	6	10	NULL	0	NULL	hydrophobic contact	NULL		stabilize	NULL		Phe96A-Phe96B		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_6115_s_277	14600147	2  The hydrophobic contact Phe96A-Phe96B remains and apparently contributes to stabilizing the ANP-bound activated complex.	bind
44710	1	6923	6	10	NULL	0	NULL	ANP	NULL		bind	NULL				activated complex	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_6115_s_277	14600147	2  The hydrophobic contact Phe96A-Phe96B remains and apparently contributes to stabilizing the ANP-bound activated complex.	bind
24970	1	6924	5	13	NULL	NULL	NULL	RTs	GP	dNTP utilization efficiency of	contributes to					host cell specificity	Process				NULL	retroviruses	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_13_12190_s_262	15644314	2  These combined findings support the idea that the dNTP utilization efficiency and dNTP binding affinity of RTs contribute to the host cell specificity of retroviruses.	bind
24971	2	6924	5	13	NULL	NULL	NULL	RTs	GP	dNTP binding affinity of	contributes to					host cell specificity	Process				NULL	retroviruses	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_13_12190_s_262	15644314	2  These combined findings support the idea that the dNTP utilization efficiency and dNTP binding affinity of RTs contribute to the host cell specificity of retroviruses.	bind
20591	1	6924	6	10	NULL	0	NULL	RTs		dNTP utilization efficiency of	contribute to					host cell specificity					NULL	retroviruses	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_13_12190_s_262	15644314	2  These combined findings support the idea that the dNTP utilization efficiency and dNTP binding affinity of RTs contribute to the host cell specificity of retroviruses.	bind
20592	2	6924	6	10	NULL	0	NULL	RTs		 dNTP binding affinity of	contribute to					host cell specificity					NULL	retroviruses	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_13_12190_s_262	15644314	2  These combined findings support the idea that the dNTP utilization efficiency and dNTP binding affinity of RTs contribute to the host cell specificity of retroviruses.	bind
24972	1	6925	5	13	NULL	NULL	NULL	tissue factor	GP		bind					factor VII/VIIa	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_22_2651_s_19	10840019	2  Tissue factor binds factor VII/VIIa, and the TF:VIIa complex can proteolytically activate factor X, which in turn activates thrombin and generates fibrin.	bind
24973	2	6925	5	13	NULL	NULL	NULL	TF:VIIa complex	GP		activates		proteolytically			factor X	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_22_2651_s_19	10840019	2  Tissue factor binds factor VII/VIIa, and the TF:VIIa complex can proteolytically activate factor X, which in turn activates thrombin and generates fibrin.	bind
24974	3	6925	5	13	NULL	NULL	NULL	factor X	GP	activated	activates					thrombin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_22_2651_s_19	10840019	2  Tissue factor binds factor VII/VIIa, and the TF:VIIa complex can proteolytically activate factor X, which in turn activates thrombin and generates fibrin.	bind
24975	4	6925	5	13	NULL	NULL	NULL	statement 3	Process		generates					fibrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_22_2651_s_19	10840019	2  Tissue factor binds factor VII/VIIa, and the TF:VIIa complex can proteolytically activate factor X, which in turn activates thrombin and generates fibrin.	bind
20593	1	6925	6	NULL	NULL	0	NULL	Tissue factor	NULL		bind	NULL				factor VII/VIIa	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_101_22_2651_s_19	10840019	2  Tissue factor binds factor VII/VIIa, and the TF:VIIa complex can proteolytically activate factor X, which in turn activates thrombin and generates fibrin.	bind
20594	2	6925	6	10	NULL	0	NULL	TF:VIIa complex			activate		proteolytically			factor X					NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_22_2651_s_19	10840019	2  Tissue factor binds factor VII/VIIa, and the TF:VIIa complex can proteolytically activate factor X, which in turn activates thrombin and generates fibrin.	bind
20595	3	6925	6	NULL	NULL	0	NULL	factor X	NULL	activated	activates	NULL				thrombin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_101_22_2651_s_19	10840019	2  Tissue factor binds factor VII/VIIa, and the TF:VIIa complex can proteolytically activate factor X, which in turn activates thrombin and generates fibrin.	bind
20596	4	6925	6	NULL	NULL	0	NULL	statement 3	NULL		generates	NULL				fibrin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_101_22_2651_s_19	10840019	2  Tissue factor binds factor VII/VIIa, and the TF:VIIa complex can proteolytically activate factor X, which in turn activates thrombin and generates fibrin.	bind
25145	1	6926	5	13	NULL	NULL	NULL	CREB	GP		bind									AP-1 site 	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_17_10647_s_306	9553127	2 (iii) Whether CREB or ATF-1 binds to the AP-1 site in a gel shift, this protein was not phosphorylated in response to PTH, since anti-phospho-CREB antibody did not cause a supershift (Fig.  7), whereas we know this antibody will supershift PTH-induced phosphorylated CREB bound to a cyclic AMP-response element in the c- fos gene ( 24).	bind
25146	2	6926	5	13	NULL	NULL	NULL	CREB	GP	PTH-induced phosphorylated	bind					c- fos gene	GP			cyclic AMP-response element	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_17_10647_s_306	9553127	2 (iii) Whether CREB or ATF-1 binds to the AP-1 site in a gel shift, this protein was not phosphorylated in response to PTH, since anti-phospho-CREB antibody did not cause a supershift (Fig.  7), whereas we know this antibody will supershift PTH-induced phosphorylated CREB bound to a cyclic AMP-response element in the c- fos gene ( 24).	bind
25147	3	6926	5	13	NULL	NULL	NULL	ATF-1	GP		bind									AP-1 site 	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_17_10647_s_306	9553127	2 (iii) Whether CREB or ATF-1 binds to the AP-1 site in a gel shift, this protein was not phosphorylated in response to PTH, since anti-phospho-CREB antibody did not cause a supershift (Fig.  7), whereas we know this antibody will supershift PTH-induced phosphorylated CREB bound to a cyclic AMP-response element in the c- fos gene ( 24).	bind
20597	1	6926	6	NULL	NULL	0	NULL	CREB	NULL		bind	NULL					NULL			AP-1 site	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_17_10647_s_306	9553127	2 (iii) Whether CREB or ATF-1 binds to the AP-1 site in a gel shift, this protein was not phosphorylated in response to PTH, since anti-phospho-CREB antibody did not cause a supershift (Fig.  7), whereas we know this antibody will supershift PTH-induced phosphorylated CREB bound to a cyclic AMP-response element in the c- fos gene ( 24).	bind
20598	2	6926	6	NULL	NULL	0	NULL	ATF-1	NULL		bind	NULL					NULL			AP-1 site	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_17_10647_s_306	9553127	2 (iii) Whether CREB or ATF-1 binds to the AP-1 site in a gel shift, this protein was not phosphorylated in response to PTH, since anti-phospho-CREB antibody did not cause a supershift (Fig.  7), whereas we know this antibody will supershift PTH-induced phosphorylated CREB bound to a cyclic AMP-response element in the c- fos gene ( 24).	bind
20736	3	6926	6	NULL	NULL	0	NULL	CREB	NULL	PTH-induced phosphorylated	bind	NULL				c-fos gene	NULL			cyclic AMP-response element	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_17_10647_s_306	9553127	2 (iii) Whether CREB or ATF-1 binds to the AP-1 site in a gel shift, this protein was not phosphorylated in response to PTH, since anti-phospho-CREB antibody did not cause a supershift (Fig.  7), whereas we know this antibody will supershift PTH-induced phosphorylated CREB bound to a cyclic AMP-response element in the c- fos gene ( 24).	bind
25148	1	6927	5	13	NULL	NULL	NULL	fibrinogen	GP	circulating	bind					GP IIb/IIa	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_4_399_s_19	11468200	2 -  6 These agents block the binding of circulating fibrinogen and von Willebrand factor to GP IIb/IIa, preventing the cross-linking of platelets necessary for aggregation and thrombosis.	bind
25149	2	6927	5	13	NULL	NULL	NULL	von Willebrand factor	GP		bind					GP IIb/IIa	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_4_399_s_19	11468200	2 -  6 These agents block the binding of circulating fibrinogen and von Willebrand factor to GP IIb/IIa, preventing the cross-linking of platelets necessary for aggregation and thrombosis.	bind
25150	3	6927	5	13	NULL	NULL	NULL	platelets	Cell		is necessary for					aggregation	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_4_399_s_19	11468200	2 -  6 These agents block the binding of circulating fibrinogen and von Willebrand factor to GP IIb/IIa, preventing the cross-linking of platelets necessary for aggregation and thrombosis.	bind
25151	4	6927	5	13	NULL	NULL	NULL	platelets	Cell		is necessary for					thrombosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_4_399_s_19	11468200	2 -  6 These agents block the binding of circulating fibrinogen and von Willebrand factor to GP IIb/IIa, preventing the cross-linking of platelets necessary for aggregation and thrombosis.	bind
25152	5	6927	5	13	NULL	NULL	NULL	statement 1	Process	blocking of	prevents					statement 3	Process	cross-linking of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_4_399_s_19	11468200	2 -  6 These agents block the binding of circulating fibrinogen and von Willebrand factor to GP IIb/IIa, preventing the cross-linking of platelets necessary for aggregation and thrombosis.	bind
25153	6	6927	5	13	NULL	NULL	NULL	statement 1	Process	blocking of	prevents					statement 4	Process	cross-linking of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_4_399_s_19	11468200	2 -  6 These agents block the binding of circulating fibrinogen and von Willebrand factor to GP IIb/IIa, preventing the cross-linking of platelets necessary for aggregation and thrombosis.	bind
25154	7	6927	5	13	NULL	NULL	NULL	statement 2	Process	blocking of	prevents					statement 3	Process	cross-linking of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_4_399_s_19	11468200	2 -  6 These agents block the binding of circulating fibrinogen and von Willebrand factor to GP IIb/IIa, preventing the cross-linking of platelets necessary for aggregation and thrombosis.	bind
25155	8	6927	5	13	NULL	NULL	NULL	statement 2	Process	blocking of	prevents					statement 4	Process	cross-linking of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_4_399_s_19	11468200	2 -  6 These agents block the binding of circulating fibrinogen and von Willebrand factor to GP IIb/IIa, preventing the cross-linking of platelets necessary for aggregation and thrombosis.	bind
20599	1	6927	6	NULL	NULL	0	NULL	fibrinogen	NULL	circulating	bind	NULL				GP IIb/IIa	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_104_4_399_s_19	11468200	2 -  6 These agents block the binding of circulating fibrinogen and von Willebrand factor to GP IIb/IIa, preventing the cross-linking of platelets necessary for aggregation and thrombosis.	bind
20600	2	6927	6	NULL	NULL	0	NULL	von Willebrand factor	NULL		bind	NULL				GP IIb/IIa	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_104_4_399_s_19	11468200	2 -  6 These agents block the binding of circulating fibrinogen and von Willebrand factor to GP IIb/IIa, preventing the cross-linking of platelets necessary for aggregation and thrombosis.	bind
30675	3	6927	6	NULL	NULL	0	NULL	platelets	NULL		is necessary for	NULL				aggregation	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_104_4_399_s_19	11468200	2 -  6 These agents block the binding of circulating fibrinogen and von Willebrand factor to GP IIb/IIa, preventing the cross-linking of platelets necessary for aggregation and thrombosis.	bind
30676	4	6927	6	NULL	NULL	0	NULL	platelets	NULL		is necessary for	NULL				thrombosis	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_104_4_399_s_19	11468200	2 -  6 These agents block the binding of circulating fibrinogen and von Willebrand factor to GP IIb/IIa, preventing the cross-linking of platelets necessary for aggregation and thrombosis.	bind
30677	5	6927	6	NULL	NULL	0	NULL	statement 1	NULL	blocking of	prevents	NULL				statement 3	NULL	cross-linking of			NULL		0	NULL	NULL	NULL	gw60_circulation_104_4_399_s_19	11468200	2 -  6 These agents block the binding of circulating fibrinogen and von Willebrand factor to GP IIb/IIa, preventing the cross-linking of platelets necessary for aggregation and thrombosis.	bind
30678	6	6927	6	NULL	NULL	0	NULL	statement 1	NULL	blocking of	prevents	NULL				statement 4	NULL	cross-linking of			NULL		0	NULL	NULL	NULL	gw60_circulation_104_4_399_s_19	11468200	2 -  6 These agents block the binding of circulating fibrinogen and von Willebrand factor to GP IIb/IIa, preventing the cross-linking of platelets necessary for aggregation and thrombosis.	bind
30679	7	6927	6	NULL	NULL	0	NULL	statement 2	NULL	blocking of	prevents	NULL				statement 3	NULL	cross-linking of			NULL		0	NULL	NULL	NULL	gw60_circulation_104_4_399_s_19	11468200	2 -  6 These agents block the binding of circulating fibrinogen and von Willebrand factor to GP IIb/IIa, preventing the cross-linking of platelets necessary for aggregation and thrombosis.	bind
30680	8	6927	6	NULL	NULL	0	NULL	statement 2	NULL	blocking of	prevents	NULL				statement 4	NULL	cross-linking of			NULL		0	NULL	NULL	NULL	gw60_circulation_104_4_399_s_19	11468200	2 -  6 These agents block the binding of circulating fibrinogen and von Willebrand factor to GP IIb/IIa, preventing the cross-linking of platelets necessary for aggregation and thrombosis.	bind
25156	1	6928	5	13	NULL	NULL	NULL	GEFs	GP		is					guanine nucleotide exchange factors	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_12_1296_s_16	16269655	2 - 4   Epac proteins are guanine nucleotide exchange factors (GEFs) that bind cAMP with affinities similar to that of the regulatory subunit of PKA. 2,3  They have been shown to function as GEFs for the Ras-like small GTPases Rap1 and Rap2 and are directly activated by cAMP in a PKA independent manner.	bind
25157	2	6928	5	13	NULL	NULL	NULL	Epac proteins	GP		bind					cAMP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_12_1296_s_16	16269655	2 - 4   Epac proteins are guanine nucleotide exchange factors (GEFs) that bind cAMP with affinities similar to that of the regulatory subunit of PKA. 2,3  They have been shown to function as GEFs for the Ras-like small GTPases Rap1 and Rap2 and are directly activated by cAMP in a PKA independent manner.	bind
25158	3	6928	5	13	NULL	NULL	NULL	Epac proteins	GP		bind					PKA	GP		regulatory subunit		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_12_1296_s_16	16269655	2 - 4   Epac proteins are guanine nucleotide exchange factors (GEFs) that bind cAMP with affinities similar to that of the regulatory subunit of PKA. 2,3  They have been shown to function as GEFs for the Ras-like small GTPases Rap1 and Rap2 and are directly activated by cAMP in a PKA independent manner.	bind
25159	4	6928	5	13	NULL	NULL	NULL	statement 2	Process		similar affinity as					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_12_1296_s_16	16269655	2 - 4   Epac proteins are guanine nucleotide exchange factors (GEFs) that bind cAMP with affinities similar to that of the regulatory subunit of PKA. 2,3  They have been shown to function as GEFs for the Ras-like small GTPases Rap1 and Rap2 and are directly activated by cAMP in a PKA independent manner.	bind
25160	5	6928	5	13	NULL	NULL	NULL	Epac proteins	GP		function as					GEFs	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_12_1296_s_16	16269655	2 - 4   Epac proteins are guanine nucleotide exchange factors (GEFs) that bind cAMP with affinities similar to that of the regulatory subunit of PKA. 2,3  They have been shown to function as GEFs for the Ras-like small GTPases Rap1 and Rap2 and are directly activated by cAMP in a PKA independent manner.	bind
25161	6	6928	5	13	NULL	NULL	NULL	statement 5	GP		occurs for					Rap1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_12_1296_s_16	16269655	2 - 4   Epac proteins are guanine nucleotide exchange factors (GEFs) that bind cAMP with affinities similar to that of the regulatory subunit of PKA. 2,3  They have been shown to function as GEFs for the Ras-like small GTPases Rap1 and Rap2 and are directly activated by cAMP in a PKA independent manner.	bind
25162	7	6928	5	13	NULL	NULL	NULL	statement 5	GP		occurs for					Rap2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_12_1296_s_16	16269655	2 - 4   Epac proteins are guanine nucleotide exchange factors (GEFs) that bind cAMP with affinities similar to that of the regulatory subunit of PKA. 2,3  They have been shown to function as GEFs for the Ras-like small GTPases Rap1 and Rap2 and are directly activated by cAMP in a PKA independent manner.	bind
25163	8	6928	5	13	NULL	NULL	NULL	Epac proteins	GP		is activated by		directly			cAMP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_12_1296_s_16	16269655	2 - 4   Epac proteins are guanine nucleotide exchange factors (GEFs) that bind cAMP with affinities similar to that of the regulatory subunit of PKA. 2,3  They have been shown to function as GEFs for the Ras-like small GTPases Rap1 and Rap2 and are directly activated by cAMP in a PKA independent manner.	bind
25164	9	6928	5	13	NULL	NULL	NULL	statement 8	Process		is independent of					PKA	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_12_1296_s_16	16269655	2 - 4   Epac proteins are guanine nucleotide exchange factors (GEFs) that bind cAMP with affinities similar to that of the regulatory subunit of PKA. 2,3  They have been shown to function as GEFs for the Ras-like small GTPases Rap1 and Rap2 and are directly activated by cAMP in a PKA independent manner.	bind
44750	10	6928	5	13	NULL	NULL	NULL	Rap1	GP		is a type of					Ras-like small GTPases	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_12_1296_s_16	16269655	2 - 4   Epac proteins are guanine nucleotide exchange factors (GEFs) that bind cAMP with affinities similar to that of the regulatory subunit of PKA. 2,3  They have been shown to function as GEFs for the Ras-like small GTPases Rap1 and Rap2 and are directly activated by cAMP in a PKA independent manner.	bind
44751	11	6928	5	13	NULL	NULL	NULL	Rap2	GP		is a type of					Ras-like small GTPases	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_12_1296_s_16	16269655	2 - 4   Epac proteins are guanine nucleotide exchange factors (GEFs) that bind cAMP with affinities similar to that of the regulatory subunit of PKA. 2,3  They have been shown to function as GEFs for the Ras-like small GTPases Rap1 and Rap2 and are directly activated by cAMP in a PKA independent manner.	bind
20601	1	6928	6	10	NULL	0	NULL	Epac proteins			is a type of					GEF					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_12_1296_s_16	16269655	2 - 4   Epac proteins are guanine nucleotide exchange factors (GEFs) that bind cAMP with affinities similar to that of the regulatory subunit of PKA. 2,3  They have been shown to function as GEFs for the Ras-like small GTPases Rap1 and Rap2 and are directly activated by cAMP in a PKA independent manner.	bind
20602	2	6928	6	NULL	NULL	0	NULL	GEF	NULL		is	NULL				guanine nucleotide exchange factor	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_12_1296_s_16	16269655	2 - 4   Epac proteins are guanine nucleotide exchange factors (GEFs) that bind cAMP with affinities similar to that of the regulatory subunit of PKA. 2,3  They have been shown to function as GEFs for the Ras-like small GTPases Rap1 and Rap2 and are directly activated by cAMP in a PKA independent manner.	bind
20603	3	6928	6	NULL	NULL	0	NULL	Epac proteins	NULL		bind	NULL				cAMP	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_12_1296_s_16	16269655	2 - 4   Epac proteins are guanine nucleotide exchange factors (GEFs) that bind cAMP with affinities similar to that of the regulatory subunit of PKA. 2,3  They have been shown to function as GEFs for the Ras-like small GTPases Rap1 and Rap2 and are directly activated by cAMP in a PKA independent manner.	bind
20604	4	6928	6	NULL	NULL	0	NULL	PKA	NULL		bind	NULL		regulatory subunit		cAMP	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_12_1296_s_16	16269655	2 - 4   Epac proteins are guanine nucleotide exchange factors (GEFs) that bind cAMP with affinities similar to that of the regulatory subunit of PKA. 2,3  They have been shown to function as GEFs for the Ras-like small GTPases Rap1 and Rap2 and are directly activated by cAMP in a PKA independent manner.	bind
20605	5	6928	6	NULL	NULL	0	NULL	statement 3	NULL		is of similar affinity as	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_12_1296_s_16	16269655	2 - 4   Epac proteins are guanine nucleotide exchange factors (GEFs) that bind cAMP with affinities similar to that of the regulatory subunit of PKA. 2,3  They have been shown to function as GEFs for the Ras-like small GTPases Rap1 and Rap2 and are directly activated by cAMP in a PKA independent manner.	bind
20606	6	6928	6	NULL	NULL	0	NULL	cAMP	NULL		activates	NULL	directly			Epac proteins	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_12_1296_s_16	16269655	2 - 4   Epac proteins are guanine nucleotide exchange factors (GEFs) that bind cAMP with affinities similar to that of the regulatory subunit of PKA. 2,3  They have been shown to function as GEFs for the Ras-like small GTPases Rap1 and Rap2 and are directly activated by cAMP in a PKA independent manner.	bind
20607	7	6928	6	NULL	NULL	0	NULL	statement 6	NULL		is independent of	NULL				PKA	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_12_1296_s_16	16269655	2 - 4   Epac proteins are guanine nucleotide exchange factors (GEFs) that bind cAMP with affinities similar to that of the regulatory subunit of PKA. 2,3  They have been shown to function as GEFs for the Ras-like small GTPases Rap1 and Rap2 and are directly activated by cAMP in a PKA independent manner.	bind
20608	8	6928	6	NULL	NULL	0	NULL	statement 1	NULL		occurs for	NULL				Rap1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_12_1296_s_16	16269655	2 - 4   Epac proteins are guanine nucleotide exchange factors (GEFs) that bind cAMP with affinities similar to that of the regulatory subunit of PKA. 2,3  They have been shown to function as GEFs for the Ras-like small GTPases Rap1 and Rap2 and are directly activated by cAMP in a PKA independent manner.	bind
20609	9	6928	6	NULL	NULL	0	NULL	statement 1	NULL		occurs for	NULL				Rap2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_12_1296_s_16	16269655	2 - 4   Epac proteins are guanine nucleotide exchange factors (GEFs) that bind cAMP with affinities similar to that of the regulatory subunit of PKA. 2,3  They have been shown to function as GEFs for the Ras-like small GTPases Rap1 and Rap2 and are directly activated by cAMP in a PKA independent manner.	bind
20610	10	6928	6	10	NULL	0	NULL	Rap1	NULL		is a type of	NULL				Ras-like small GTPases	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_12_1296_s_16	16269655	2 - 4   Epac proteins are guanine nucleotide exchange factors (GEFs) that bind cAMP with affinities similar to that of the regulatory subunit of PKA. 2,3  They have been shown to function as GEFs for the Ras-like small GTPases Rap1 and Rap2 and are directly activated by cAMP in a PKA independent manner.	bind
20611	11	6928	6	10	NULL	0	NULL	Rap2	NULL		is a type of	NULL				Ras-like small GTPases	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_12_1296_s_16	16269655	2 - 4   Epac proteins are guanine nucleotide exchange factors (GEFs) that bind cAMP with affinities similar to that of the regulatory subunit of PKA. 2,3  They have been shown to function as GEFs for the Ras-like small GTPases Rap1 and Rap2 and are directly activated by cAMP in a PKA independent manner.	bind
25165	1	6929	5	13	NULL	NULL	NULL	PDGF	GP		bind		selectively	A chain		alpha PDGFR	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_787_s_21	15061151	2 - 4   The PDGF A and C chains selectively bind alpha PDGFR, whereas PDGF D preferentially binds beta PDGFR and PDGF B displays similar affinity for both receptors.	bind
25166	2	6929	5	13	NULL	NULL	NULL	PDGF	GP		bind		selectively	C chain		alpha PDGFR	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_787_s_21	15061151	2 - 4   The PDGF A and C chains selectively bind alpha PDGFR, whereas PDGF D preferentially binds beta PDGFR and PDGF B displays similar affinity for both receptors.	bind
25167	3	6929	5	13	NULL	NULL	NULL	PDGF	GP		bind		preferentially	D chain		beta PDGFR	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_787_s_21	15061151	2 - 4   The PDGF A and C chains selectively bind alpha PDGFR, whereas PDGF D preferentially binds beta PDGFR and PDGF B displays similar affinity for both receptors.	bind
25168	4	6929	5	13	NULL	NULL	NULL	PDGF	GP		bind			B chain		alpha PDGFR	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_787_s_21	15061151	2 - 4   The PDGF A and C chains selectively bind alpha PDGFR, whereas PDGF D preferentially binds beta PDGFR and PDGF B displays similar affinity for both receptors.	bind
25169	5	6929	5	13	NULL	NULL	NULL	PDGF	GP		bind			B chain		beta PDGFR	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_787_s_21	15061151	2 - 4   The PDGF A and C chains selectively bind alpha PDGFR, whereas PDGF D preferentially binds beta PDGFR and PDGF B displays similar affinity for both receptors.	bind
25170	6	6929	5	13	NULL	NULL	NULL	statement 4	Process		similar affinity as					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_787_s_21	15061151	2 - 4   The PDGF A and C chains selectively bind alpha PDGFR, whereas PDGF D preferentially binds beta PDGFR and PDGF B displays similar affinity for both receptors.	bind
20612	1	6929	6	NULL	NULL	0	NULL	PDGF	NULL		bind	NULL	selectively	A chain		alpha PDGFR	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_787_s_21	15061151	2 - 4   The PDGF A and C chains selectively bind alpha PDGFR, whereas PDGF D preferentially binds beta PDGFR and PDGF B displays similar affinity for both receptors.	bind
20613	2	6929	6	NULL	NULL	0	NULL	PDGF	NULL		bind	NULL	selectively	C chain		alpha PDGFR	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_787_s_21	15061151	2 - 4   The PDGF A and C chains selectively bind alpha PDGFR, whereas PDGF D preferentially binds beta PDGFR and PDGF B displays similar affinity for both receptors.	bind
20614	3	6929	6	NULL	NULL	0	NULL	PDGF	NULL		bind	NULL	preferentially	D chain		beta PDGFR	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_787_s_21	15061151	2 - 4   The PDGF A and C chains selectively bind alpha PDGFR, whereas PDGF D preferentially binds beta PDGFR and PDGF B displays similar affinity for both receptors.	bind
20615	4	6929	6	NULL	NULL	0	NULL	PDGF	NULL		bind	NULL		B chain		alpha PDGFR	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_787_s_21	15061151	2 - 4   The PDGF A and C chains selectively bind alpha PDGFR, whereas PDGF D preferentially binds beta PDGFR and PDGF B displays similar affinity for both receptors.	bind
20616	5	6929	6	NULL	NULL	0	NULL	PDGF 	NULL		bind	NULL		B chain		beta PDGFR	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_787_s_21	15061151	2 - 4   The PDGF A and C chains selectively bind alpha PDGFR, whereas PDGF D preferentially binds beta PDGFR and PDGF B displays similar affinity for both receptors.	bind
20617	6	6929	6	NULL	NULL	0	NULL	statement 4	NULL		has equal affinity as	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_787_s_21	15061151	2 - 4   The PDGF A and C chains selectively bind alpha PDGFR, whereas PDGF D preferentially binds beta PDGFR and PDGF B displays similar affinity for both receptors.	bind
25171	1	6930	5	13	NULL	NULL	NULL	Cx43	GP		bind					c-Src	GP	constitutively active			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_2_215_s_19	14699011	2 - 5    Recent studies show that this association is potentially interlinked, because binding of Cx43 to constitutively active c-Src is correlated with a decrease in the Cx43/ZO-1 interaction.	bind
25172	3	6930	5	13	NULL	NULL	NULL	statement 1	Process		correlates with					statement 2	Process	decrease in			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_2_215_s_19	14699011	2 - 5    Recent studies show that this association is potentially interlinked, because binding of Cx43 to constitutively active c-Src is correlated with a decrease in the Cx43/ZO-1 interaction.	bind
31485	2	6930	5	13	NULL	NULL	NULL	Cx43	GP		interacts with					ZO-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_2_215_s_19	14699011	2 - 5    Recent studies show that this association is potentially interlinked, because binding of Cx43 to constitutively active c-Src is correlated with a decrease in the Cx43/ZO-1 interaction.	bind
20618	1	6930	6	NULL	NULL	0	NULL	Cx43	NULL		bind	NULL				c-Src	NULL	constitutively active			NULL		0	NULL	NULL	NULL	gw70_circulationres_94_2_215_s_19	14699011	2 - 5    Recent studies show that this association is potentially interlinked, because binding of Cx43 to constitutively active c-Src is correlated with a decrease in the Cx43/ZO-1 interaction.	bind
20619	2	6930	6	NULL	NULL	0	NULL	Cx43	NULL		interacts with	NULL				ZO-1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_2_215_s_19	14699011	2 - 5    Recent studies show that this association is potentially interlinked, because binding of Cx43 to constitutively active c-Src is correlated with a decrease in the Cx43/ZO-1 interaction.	bind
20620	3	6930	6	NULL	NULL	0	NULL	statement 1	NULL		correlates with	NULL				statement 2	NULL	decrease in			NULL		0	NULL	NULL	NULL	gw70_circulationres_94_2_215_s_19	14699011	2 - 5    Recent studies show that this association is potentially interlinked, because binding of Cx43 to constitutively active c-Src is correlated with a decrease in the Cx43/ZO-1 interaction.	bind
25173	1	6931	5	13	NULL	NULL	NULL	2 -F-arabino-FAD	GP		bind		very tightly			apo-glucose oxidase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_33_19915_s_225	8702705	2 -F-arabino-FAD binds very tightly to apo-glucose oxidase with quenching of the fluorescence and changes in the lambdamax from 372 and 444 nm to 376 and 454 nm.	bind
20621	1	6931	6	NULL	NULL	0	NULL	F-arabino-FAD	NULL		bind	NULL	very tightly			apo-glucose oxidase 	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_33_19915_s_225	8702705	2 -F-arabino-FAD binds very tightly to apo-glucose oxidase with quenching of the fluorescence and changes in the lambdamax from 372 and 444 nm to 376 and 454 nm.	bind
25174	1	6933	5	13	NULL	NULL	NULL	LIFR	GP		is					LIF-specific receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_7_787_s_19	10764413	2 3  LIF binds to a receptor complex consisting of a LIF-specific receptor (LIFR) and the signal transducer gp130.	bind
25175	2	6933	5	13	NULL	NULL	NULL	LIFR	GP		is in complex with					gp130	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_7_787_s_19	10764413	2 3  LIF binds to a receptor complex consisting of a LIF-specific receptor (LIFR) and the signal transducer gp130.	bind
25176	3	6933	5	13	NULL	NULL	NULL	LIF	GP		bind					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_7_787_s_19	10764413	2 3  LIF binds to a receptor complex consisting of a LIF-specific receptor (LIFR) and the signal transducer gp130.	bind
31486	4	6933	5	13	NULL	NULL	NULL	gp130	GP		is a type of					signal transducer	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_7_787_s_19	10764413	2 3  LIF binds to a receptor complex consisting of a LIF-specific receptor (LIFR) and the signal transducer gp130.	bind
20622	1	6933	6	NULL	NULL	0	NULL	LIF-specifc receptor	NULL		forms a complex with	NULL				gp130	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_86_7_787_s_19	10764413	2 3  LIF binds to a receptor complex consisting of a LIF-specific receptor (LIFR) and the signal transducer gp130.	bind
20623	2	6933	6	NULL	NULL	0	NULL	LIFR	NULL		is	NULL				LIF-specific receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_86_7_787_s_19	10764413	2 3  LIF binds to a receptor complex consisting of a LIF-specific receptor (LIFR) and the signal transducer gp130.	bind
20624	3	6933	6	NULL	NULL	0	NULL	gp130	NULL		is a type of	NULL				signal transducer	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_7_787_s_19	10764413	2 3  LIF binds to a receptor complex consisting of a LIF-specific receptor (LIFR) and the signal transducer gp130.	bind
20626	4	6933	6	NULL	NULL	0	NULL	LIF	NULL		bind	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_86_7_787_s_19	10764413	2 3  LIF binds to a receptor complex consisting of a LIF-specific receptor (LIFR) and the signal transducer gp130.	bind
25177	1	6934	5	13	NULL	NULL	NULL	Ang II	GP		bind					AT1 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_81_4_550_s_17	9314836	2 3  Nonetheless, binding of Ang II to the AT1 receptor elicits many of the same cellular events induced by mitogens such as PDGF and EGF.	bind
25178	3	6934	5	13	NULL	NULL	NULL	statement 1	Process		elicits					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_81_4_550_s_17	9314836	2 3  Nonetheless, binding of Ang II to the AT1 receptor elicits many of the same cellular events induced by mitogens such as PDGF and EGF.	bind
25179	2	6934	5	13	NULL	NULL	NULL	PDGF	GP		induce					cellular events	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_81_4_550_s_17	9314836	2 3  Nonetheless, binding of Ang II to the AT1 receptor elicits many of the same cellular events induced by mitogens such as PDGF and EGF.	bind
25181	4	6934	5	13	NULL	NULL	NULL	EGF	GP		induce					cellular events	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_81_4_550_s_17	9314836	2 3  Nonetheless, binding of Ang II to the AT1 receptor elicits many of the same cellular events induced by mitogens such as PDGF and EGF.	bind
31487	6	6934	5	13	NULL	NULL	NULL	PDGF	GP		is a type of					mitogen	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_81_4_550_s_17	9314836	2 3  Nonetheless, binding of Ang II to the AT1 receptor elicits many of the same cellular events induced by mitogens such as PDGF and EGF.	bind
31488	7	6934	5	13	NULL	NULL	NULL	EGF	GP		is a type of					mitogen	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_81_4_550_s_17	9314836	2 3  Nonetheless, binding of Ang II to the AT1 receptor elicits many of the same cellular events induced by mitogens such as PDGF and EGF.	bind
44752	5	6934	5	13	NULL	NULL	NULL	statement 1	Process		elicits					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_81_4_550_s_17	9314836	2 3  Nonetheless, binding of Ang II to the AT1 receptor elicits many of the same cellular events induced by mitogens such as PDGF and EGF.	bind
20627	1	6934	6	NULL	NULL	0	NULL	Ang II	NULL		bind	NULL				AT1 receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_81_4_550_s_17	9314836	2 3  Nonetheless, binding of Ang II to the AT1 receptor elicits many of the same cellular events induced by mitogens such as PDGF and EGF.	bind
21255	2	6934	6	NULL	NULL	0	NULL	PDGF	NULL		induce	NULL				cellular events	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_81_4_550_s_17	9314836	2 3  Nonetheless, binding of Ang II to the AT1 receptor elicits many of the same cellular events induced by mitogens such as PDGF and EGF.	bind
21256	3	6934	6	NULL	NULL	0	NULL	EGF	NULL		induce	NULL				cellular events	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_81_4_550_s_17	9314836	2 3  Nonetheless, binding of Ang II to the AT1 receptor elicits many of the same cellular events induced by mitogens such as PDGF and EGF.	bind
21257	4	6934	6	NULL	NULL	0	NULL	statement 1	NULL		elicits	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_81_4_550_s_17	9314836	2 3  Nonetheless, binding of Ang II to the AT1 receptor elicits many of the same cellular events induced by mitogens such as PDGF and EGF.	bind
21258	5	6934	6	NULL	NULL	0	NULL	statement 1	NULL		elicits	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_81_4_550_s_17	9314836	2 3  Nonetheless, binding of Ang II to the AT1 receptor elicits many of the same cellular events induced by mitogens such as PDGF and EGF.	bind
30681	6	6934	6	NULL	NULL	0	NULL	PDGF	NULL		is a type of	NULL				mitogen	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_81_4_550_s_17	9314836	2 3  Nonetheless, binding of Ang II to the AT1 receptor elicits many of the same cellular events induced by mitogens such as PDGF and EGF.	bind
30682	7	6934	6	NULL	NULL	0	NULL	EGF	NULL		is a type of	NULL				mitogen	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_81_4_550_s_17	9314836	2 3  Nonetheless, binding of Ang II to the AT1 receptor elicits many of the same cellular events induced by mitogens such as PDGF and EGF.	bind
25183	1	6935	5	13	NULL	NULL	NULL	VIIa	GP		bind					TF	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_11_1333_s_15	8911271	2 3 4 5 6  VIIa bound to TF initiates blood coagulation by activating factors IX and X, 7 8 9  a process already observed in the 1960s by Josso and Prou-Wartelle 10  and Nossel.	bind
25184	2	6935	5	13	NULL	NULL	NULL	statement 1	Process		initiates					blood coagulation	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_11_1333_s_15	8911271	2 3 4 5 6  VIIa bound to TF initiates blood coagulation by activating factors IX and X, 7 8 9  a process already observed in the 1960s by Josso and Prou-Wartelle 10  and Nossel.	bind
25185	3	6935	5	13	NULL	NULL	NULL	statement 2	Process		occurs by					factor IX	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_11_1333_s_15	8911271	2 3 4 5 6  VIIa bound to TF initiates blood coagulation by activating factors IX and X, 7 8 9  a process already observed in the 1960s by Josso and Prou-Wartelle 10  and Nossel.	bind
25186	4	6935	5	13	NULL	NULL	NULL	statement 2	Process		occurs by					factor X	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_11_1333_s_15	8911271	2 3 4 5 6  VIIa bound to TF initiates blood coagulation by activating factors IX and X, 7 8 9  a process already observed in the 1960s by Josso and Prou-Wartelle 10  and Nossel.	bind
20628	1	6935	6	NULL	NULL	0	NULL	VIIa	NULL		bind	NULL				TF	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_11_1333_s_15	8911271	2 3 4 5 6  VIIa bound to TF initiates blood coagulation by activating factors IX and X, 7 8 9  a process already observed in the 1960s by Josso and Prou-Wartelle 10  and Nossel.	bind
20629	2	6935	6	NULL	NULL	0	NULL	statement 1	NULL		initiates	NULL				blood coagulation	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_11_1333_s_15	8911271	2 3 4 5 6  VIIa bound to TF initiates blood coagulation by activating factors IX and X, 7 8 9  a process already observed in the 1960s by Josso and Prou-Wartelle 10  and Nossel.	bind
20630	3	6935	6	NULL	NULL	0	NULL	statement 2	NULL		occurs by	NULL				factor IX	NULL	activation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_11_1333_s_15	8911271	2 3 4 5 6  VIIa bound to TF initiates blood coagulation by activating factors IX and X, 7 8 9  a process already observed in the 1960s by Josso and Prou-Wartelle 10  and Nossel.	bind
20631	4	6935	6	NULL	NULL	0	NULL	statement 2	NULL		occurs by	NULL				factor X	NULL	activation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_11_1333_s_15	8911271	2 3 4 5 6  VIIa bound to TF initiates blood coagulation by activating factors IX and X, 7 8 9  a process already observed in the 1960s by Josso and Prou-Wartelle 10  and Nossel.	bind
25187	1	6936	5	13	NULL	NULL	NULL	cTnT	GP		bind		high affinity	NH2-terminal half		actin-Tm	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_5_471_s_146	9734469	2 3 42  As illustrated in Figure 2   and based largely on studies with fsTnT, it is apparent that both the NH2- and COOH-terminal halves of cTnT bind to actin-Tm with high affinity.	bind
25188	2	6936	5	13	NULL	NULL	NULL	cTnT	GP		bind		high affinity	COOH-terminal half		actin-Tm	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_5_471_s_146	9734469	2 3 42  As illustrated in Figure 2   and based largely on studies with fsTnT, it is apparent that both the NH2- and COOH-terminal halves of cTnT bind to actin-Tm with high affinity.	bind
20632	1	6936	6	NULL	NULL	0	NULL	cTnT	NULL		bind	NULL	high affinity	NH2 terminus		actin-Tm	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_5_471_s_146	9734469	2 3 42  As illustrated in Figure 2   and based largely on studies with fsTnT, it is apparent that both the NH2- and COOH-terminal halves of cTnT bind to actin-Tm with high affinity.	bind
20633	2	6936	6	NULL	NULL	0	NULL	cTnT	NULL		bind	NULL	high affinity	COOH terminus		actin-Tm	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_5_471_s_146	9734469	2 3 42  As illustrated in Figure 2   and based largely on studies with fsTnT, it is apparent that both the NH2- and COOH-terminal halves of cTnT bind to actin-Tm with high affinity.	bind
25189	2	6937	5	13	NULL	NULL	NULL	fumonisin B1	Chemical	fungal	inhibits		highly specific			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_12587_s_181	11801602	2 A key enzyme in this pathway is CoA-dependent ceramide synthase, and fumonisin B1 is a highly specific fungal inhibitor of this enzyme ( 57,  58).	bind
44795	1	6937	5	13	NULL	NULL	NULL	ceramide synthase	GP		depends on					CoA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_12587_s_181	11801602	2 A key enzyme in this pathway is CoA-dependent ceramide synthase, and fumonisin B1 is a highly specific fungal inhibitor of this enzyme ( 57,  58).	bind
20709	2	6937	6	10	NULL	0	NULL	fumonisin B1	NULL	fungal	inhibits	NULL	specifically			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_12587_s_181	11801602	2 A key enzyme in this pathway is CoA-dependent ceramide synthase, and fumonisin B1 is a highly specific fungal inhibitor of this enzyme ( 57,  58).	bind
44796	1	6937	6	10	NULL	0	NULL	ceramide synthase	NULL		depends on	NULL				CoA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12587_s_181	11801602	2 A key enzyme in this pathway is CoA-dependent ceramide synthase, and fumonisin B1 is a highly specific fungal inhibitor of this enzyme ( 57,  58).	bind
25190	1	6938	5	13	NULL	NULL	NULL	CHF protein	GP		bind					B- myb	GP			DRS	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_41_39015_s_289	12147683	2 A protein (CHF) that can bind the B- myb DRS has been purified ( 41); however, evidence that this binding correlates with the sequence requirements for transcriptional corepression is lacking.	bind
56717	2	6938	5	13	NULL	NULL	NULL	statement 1	Process		does not correlate					transcriptional corepression	Process	sequence requirements of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_41_39015_s_289	12147683	2 A protein (CHF) that can bind the B- myb DRS has been purified ( 41); however, evidence that this binding correlates with the sequence requirements for transcriptional corepression is lacking.	bind
20710	1	6938	6	NULL	NULL	0	NULL	CHF protein	NULL		bind	NULL				B-myb	NULL			DRS	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_41_39015_s_289	12147683	2 A protein (CHF) that can bind the B- myb DRS has been purified ( 41); however, evidence that this binding correlates with the sequence requirements for transcriptional corepression is lacking.	bind
20711	2	6938	6	NULL	NULL	0	NULL	statement 1	NULL		does not correlate	NULL				transcriptional corepression	NULL	sequence requirements of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_41_39015_s_289	12147683	2 A protein (CHF) that can bind the B- myb DRS has been purified ( 41); however, evidence that this binding correlates with the sequence requirements for transcriptional corepression is lacking.	bind
25191	1	6939	5	13	NULL	NULL	NULL	TNFR2	GP		contains			carboxyl-terminal region		T2bs-C	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_31572_s_268	16020544	2 A recent study indicated that the same carboxyl-terminal region of TNFR2 that contains T2bs-C binds to the protein tyrosine kinase Etk/mx in endothelial cells ( ).	bind
25192	2	6939	5	13	NULL	NULL	NULL	statement 1	GP		bind					Etk/mx	GP				NULL	in endothelial cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_31572_s_268	16020544	2 A recent study indicated that the same carboxyl-terminal region of TNFR2 that contains T2bs-C binds to the protein tyrosine kinase Etk/mx in endothelial cells ( ).	bind
31489	3	6939	5	13	NULL	NULL	NULL	Etk/mx	GP		is a type of					protein tyrosine kinase	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_31572_s_268	16020544	2 A recent study indicated that the same carboxyl-terminal region of TNFR2 that contains T2bs-C binds to the protein tyrosine kinase Etk/mx in endothelial cells ( ).	bind
20712	1	6939	6	NULL	NULL	0	NULL	TNFR2	NULL		contains	NULL		carboxyl-terminal region		T2bs-C	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_36_31572_s_268	16020544	2 A recent study indicated that the same carboxyl-terminal region of TNFR2 that contains T2bs-C binds to the protein tyrosine kinase Etk/mx in endothelial cells ( ).	bind
20713	2	6939	6	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL				Etk/mx	NULL				NULL	endothelial cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_31572_s_268	16020544	2 A recent study indicated that the same carboxyl-terminal region of TNFR2 that contains T2bs-C binds to the protein tyrosine kinase Etk/mx in endothelial cells ( ).	bind
20714	3	6939	6	NULL	NULL	0	NULL	Etk/mx	NULL		is a type of	NULL				protein tyrosine kinase	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_31572_s_268	16020544	2 A recent study indicated that the same carboxyl-terminal region of TNFR2 that contains T2bs-C binds to the protein tyrosine kinase Etk/mx in endothelial cells ( ).	bind
25193	1	6940	5	NULL	NULL	0	NULL		NULL		interacts with	NULL		tryptophan		
\n	NULL		tryptophan		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20337_s_305	10764747	2 A tryptophan-tryptophan interaction may also be involved in mAb 16 binding to the alpha5 subunit because the second CDR loop of the light chain of mAb 16 contains a tryptophan residue (L. Burrows, A. P. Mould, and M. J. Humphries, unpublished results).	bind
25194	2	6940	5	13	NULL	NULL	NULL	mAb 16	GP		bind								alpha5 subunit		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_27_20337_s_305	10764747	2 A tryptophan-tryptophan interaction may also be involved in mAb 16 binding to the alpha5 subunit because the second CDR loop of the light chain of mAb 16 contains a tryptophan residue (L. Burrows, A. P. Mould, and M. J. Humphries, unpublished results).	bind
25195	3	6940	5	13	NULL	NULL	NULL	statement 1	Process		be involved in		may			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_27_20337_s_305	10764747	2 A tryptophan-tryptophan interaction may also be involved in mAb 16 binding to the alpha5 subunit because the second CDR loop of the light chain of mAb 16 contains a tryptophan residue (L. Burrows, A. P. Mould, and M. J. Humphries, unpublished results).	bind
25196	4	6940	5	13	NULL	NULL	NULL	mAb 16	GP		contains			second CDR loop of light chain					tryptophan residue		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_27_20337_s_305	10764747	2 A tryptophan-tryptophan interaction may also be involved in mAb 16 binding to the alpha5 subunit because the second CDR loop of the light chain of mAb 16 contains a tryptophan residue (L. Burrows, A. P. Mould, and M. J. Humphries, unpublished results).	bind
25197	5	6940	5	13	NULL	NULL	NULL	statement 4	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_27_20337_s_305	10764747	2 A tryptophan-tryptophan interaction may also be involved in mAb 16 binding to the alpha5 subunit because the second CDR loop of the light chain of mAb 16 contains a tryptophan residue (L. Burrows, A. P. Mould, and M. J. Humphries, unpublished results).	bind
20715	1	6940	6	NULL	NULL	0	NULL	mAb 16	NULL		bind	NULL				alpha5 subunit	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20337_s_305	10764747	2 A tryptophan-tryptophan interaction may also be involved in mAb 16 binding to the alpha5 subunit because the second CDR loop of the light chain of mAb 16 contains a tryptophan residue (L. Burrows, A. P. Mould, and M. J. Humphries, unpublished results).	bind
20716	2	6940	6	10	NULL	0	NULL				interacts with			tryptophan					tryptophan		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_27_20337_s_305	10764747	2 A tryptophan-tryptophan interaction may also be involved in mAb 16 binding to the alpha5 subunit because the second CDR loop of the light chain of mAb 16 contains a tryptophan residue (L. Burrows, A. P. Mould, and M. J. Humphries, unpublished results).	bind
20717	3	6940	6	10	NULL	0	NULL	statement 2			 be involved in		may			statement 1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_27_20337_s_305	10764747	2 A tryptophan-tryptophan interaction may also be involved in mAb 16 binding to the alpha5 subunit because the second CDR loop of the light chain of mAb 16 contains a tryptophan residue (L. Burrows, A. P. Mould, and M. J. Humphries, unpublished results).	bind
20718	4	6940	6	10	NULL	0	NULL	mAb16 	NULL		contains 	NULL		second CDR loop of light chain			NULL		tryptophan residue		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_27_20337_s_305	10764747	2 A tryptophan-tryptophan interaction may also be involved in mAb 16 binding to the alpha5 subunit because the second CDR loop of the light chain of mAb 16 contains a tryptophan residue (L. Burrows, A. P. Mould, and M. J. Humphries, unpublished results).	bind
20719	5	6940	6	NULL	NULL	0	NULL	statement 3	NULL		is because of	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20337_s_305	10764747	2 A tryptophan-tryptophan interaction may also be involved in mAb 16 binding to the alpha5 subunit because the second CDR loop of the light chain of mAb 16 contains a tryptophan residue (L. Burrows, A. P. Mould, and M. J. Humphries, unpublished results).	bind
25198	1	6941	5	13	NULL	NULL	NULL	HSF	GP		bind					HSF targets	NucleicAcid	identified			NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_5169_s_67	14612437	2 According to the previously published mRNA expression data ( ), the large majority of the identified HSF targets that are bound by HSF  in vivo are induced by heat shock.	bind
25199	2	6941	5	13	NULL	NULL	NULL	heat shock	ResearchActivity		induces					statement 1	Process				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_5169_s_67	14612437	2 According to the previously published mRNA expression data ( ), the large majority of the identified HSF targets that are bound by HSF  in vivo are induced by heat shock.	bind
20720	1	6941	6	10	NULL	0	NULL	HSF			bind					 HSF targets		identified			NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_5169_s_67	14612437	2 According to the previously published mRNA expression data ( ), the large majority of the identified HSF targets that are bound by HSF  in vivo are induced by heat shock.	bind
20721	2	6941	6	NULL	NULL	0	NULL	heat shock	NULL		induces	NULL				statement 1	NULL				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_5169_s_67	14612437	2 According to the previously published mRNA expression data ( ), the large majority of the identified HSF targets that are bound by HSF  in vivo are induced by heat shock.	bind
25200	1	6942	5	13	NULL	NULL	NULL	mPER3	GP		bind					mPER1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_49_45921_s_40	11591712	2 Additionally, mPER3 binding to mPER1 or mPER2 has been shown to contribute to nuclear localization of the heterodimer ( 19).	bind
25201	2	6942	5	13	NULL	NULL	NULL	mPER3	GP		bind					mPER2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_49_45921_s_40	11591712	2 Additionally, mPER3 binding to mPER1 or mPER2 has been shown to contribute to nuclear localization of the heterodimer ( 19).	bind
25202	3	6942	5	13	NULL	NULL	NULL	statement 1	Process		is localized to					nucleus	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_49_45921_s_40	11591712	2 Additionally, mPER3 binding to mPER1 or mPER2 has been shown to contribute to nuclear localization of the heterodimer ( 19).	bind
25203	4	6942	5	13	NULL	NULL	NULL	statement 1	Process		contributes to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_49_45921_s_40	11591712	2 Additionally, mPER3 binding to mPER1 or mPER2 has been shown to contribute to nuclear localization of the heterodimer ( 19).	bind
25204	5	6942	5	13	NULL	NULL	NULL	statement 2	Process		is localized to					nucleus	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_49_45921_s_40	11591712	2 Additionally, mPER3 binding to mPER1 or mPER2 has been shown to contribute to nuclear localization of the heterodimer ( 19).	bind
25205	6	6942	5	13	NULL	NULL	NULL	statement 2	Process		contributes to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_49_45921_s_40	11591712	2 Additionally, mPER3 binding to mPER1 or mPER2 has been shown to contribute to nuclear localization of the heterodimer ( 19).	bind
20722	1	6942	6	NULL	NULL	0	NULL	mPER3	NULL		bind	NULL				mPER1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_49_45921_s_40	11591712	2 Additionally, mPER3 binding to mPER1 or mPER2 has been shown to contribute to nuclear localization of the heterodimer ( 19).	bind
20723	2	6942	6	NULL	NULL	0	NULL	mPER3	NULL		bind	NULL				mPER2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_49_45921_s_40	11591712	2 Additionally, mPER3 binding to mPER1 or mPER2 has been shown to contribute to nuclear localization of the heterodimer ( 19).	bind
20724	3	6942	6	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_49_45921_s_40	11591712	2 Additionally, mPER3 binding to mPER1 or mPER2 has been shown to contribute to nuclear localization of the heterodimer ( 19).	bind
20725	4	6942	6	NULL	NULL	0	NULL	statement 1	NULL		localizes to	NULL				nucleus	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_49_45921_s_40	11591712	2 Additionally, mPER3 binding to mPER1 or mPER2 has been shown to contribute to nuclear localization of the heterodimer ( 19).	bind
20726	5	6942	6	NULL	NULL	0	NULL	statement 1	NULL		contribute to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_49_45921_s_40	11591712	2 Additionally, mPER3 binding to mPER1 or mPER2 has been shown to contribute to nuclear localization of the heterodimer ( 19).	bind
20727	7	6942	6	10	NULL	0	NULL	statement 2			contribute to					statement 6					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_49_45921_s_40	11591712	2 Additionally, mPER3 binding to mPER1 or mPER2 has been shown to contribute to nuclear localization of the heterodimer ( 19).	bind
31180	6	6942	6	10	NULL	0	NULL	statement 2			localizes to					nucleus					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_49_45921_s_40	11591712	2 Additionally, mPER3 binding to mPER1 or mPER2 has been shown to contribute to nuclear localization of the heterodimer ( 19).	bind
56718	7	6942	6	10	NULL	0	NULL	statement 1			is an alternative to					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_49_45921_s_40	11591712	2 Additionally, mPER3 binding to mPER1 or mPER2 has been shown to contribute to nuclear localization of the heterodimer ( 19).	bind
25206	1	6943	5	13	NULL	NULL	NULL	GR	GP		bind		intrinsically rapidly							GRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_43_39885_s_184	11518712	2 Additionally, we show that GR binding to a GRE is intrinsically rapid but can be altered by association with accessory factors.	bind
25207	3	6943	5	13	NULL	NULL	NULL	statement 2	Process		alters					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_43_39885_s_184	11518712	2 Additionally, we show that GR binding to a GRE is intrinsically rapid but can be altered by association with accessory factors.	bind
31490	2	6943	5	13	NULL	NULL	NULL	statement 1	Process		associate with					accessory factors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_43_39885_s_184	11518712	2 Additionally, we show that GR binding to a GRE is intrinsically rapid but can be altered by association with accessory factors.	bind
20728	1	6943	6	13	NULL	NULL	NULL	GR	GP		bind		intrinsically rapidly							GRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_43_39885_s_184	11518712	2 Additionally, we show that GR binding to a GRE is intrinsically rapid but can be altered by association with accessory factors.	bind
30683	2	6943	6	NULL	NULL	0	NULL	statement 1	NULL		associates with	NULL				accessory factors	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_43_39885_s_184	11518712	2 Additionally, we show that GR binding to a GRE is intrinsically rapid but can be altered by association with accessory factors.	bind
30684	3	6943	6	NULL	NULL	0	NULL	statement 2	NULL		alters	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_43_39885_s_184	11518712	2 Additionally, we show that GR binding to a GRE is intrinsically rapid but can be altered by association with accessory factors.	bind
25208	1	6944	5	13	NULL	NULL	NULL	ADP	Chemical		bind					DnaK	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_12_6643_s_401	9506960	2 ADP and Pi bind to DnaK with  K d values of 0.13 and 0.45 muM, respectively ( 19).	bind
25209	2	6944	5	13	NULL	NULL	NULL	Pi	Chemical		bind					DnaK	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_12_6643_s_401	9506960	2 ADP and Pi bind to DnaK with  K d values of 0.13 and 0.45 muM, respectively ( 19).	bind
20729	1	6944	6	NULL	NULL	0	NULL	ADP	NULL		bind	NULL				DnaK	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_12_6643_s_401	9506960	2 ADP and Pi bind to DnaK with  K d values of 0.13 and 0.45 muM, respectively ( 19).	bind
20730	2	6944	6	NULL	NULL	0	NULL	Pi	NULL		bind	NULL				DnaK	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_12_6643_s_401	9506960	2 ADP and Pi bind to DnaK with  K d values of 0.13 and 0.45 muM, respectively ( 19).	bind
25210	1	6945	5	13	NULL	NULL	NULL	actin-binding proteins	GP		bind		selectively			ATP-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_48_33827_s_174	10567336	2 Although no direct evidence exists for different structures of actin depending on bound nucleotide, it is remarkable that a number of actin-binding proteins display selective binding to either ATP- or ADP-actin.	bind
25211	2	6945	5	13	NULL	NULL	NULL	actin-binding proteins	GP		bind		selectively			ADP-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_48_33827_s_174	10567336	2 Although no direct evidence exists for different structures of actin depending on bound nucleotide, it is remarkable that a number of actin-binding proteins display selective binding to either ATP- or ADP-actin.	bind
25212	3	6945	5	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_48_33827_s_174	10567336	2 Although no direct evidence exists for different structures of actin depending on bound nucleotide, it is remarkable that a number of actin-binding proteins display selective binding to either ATP- or ADP-actin.	bind
20778	1	6945	6	NULL	NULL	0	NULL	actin-binding proteins	NULL		bind	NULL	selectively			ATP-actin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_48_33827_s_174	10567336	2 Although no direct evidence exists for different structures of actin depending on bound nucleotide, it is remarkable that a number of actin-binding proteins display selective binding to either ATP- or ADP-actin.	bind
20780	2	6945	6	NULL	NULL	0	NULL	actin-binding proteins	NULL		bind	NULL	selectively			ADP-actin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_48_33827_s_174	10567336	2 Although no direct evidence exists for different structures of actin depending on bound nucleotide, it is remarkable that a number of actin-binding proteins display selective binding to either ATP- or ADP-actin.	bind
56719	3	6945	6	10	NULL	0	NULL	statement 1			is an alternative to					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_48_33827_s_174	10567336	2 Although no direct evidence exists for different structures of actin depending on bound nucleotide, it is remarkable that a number of actin-binding proteins display selective binding to either ATP- or ADP-actin.	bind
25213	1	6947	5	13	NULL	NULL	NULL	HMG-1 peptide	GP		bind		preferentially			supercoiled DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_46_35699_s_214	10962007	2 Although transitional relieving the torsional stress in the supercoiled plasmid (without changing the linking number) by the AB didomain is not excluded (see Ref.  11), the extent of contribution of gel retardation to the "`topoisomer-like"` ladder by preferential binding of the HMG-1 peptide to supercoiled DNA (Fig.  7 c and also Ref.  21) awaits further investigation (see "`Discussion"`).	bind
20784	1	6947	6	10	NULL	0	NULL	HMG-1 peptide	NULL		bind	NULL	preferentially			supercoiled DNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_46_35699_s_214	10962007	2 Although transitional relieving the torsional stress in the supercoiled plasmid (without changing the linking number) by the AB didomain is not excluded (see Ref.  11), the extent of contribution of gel retardation to the "`topoisomer-like"` ladder by preferential binding of the HMG-1 peptide to supercoiled DNA (Fig.  7 c and also Ref.  21) awaits further investigation (see "`Discussion"`).	bind
25214	1	6948	5	13	NULL	NULL	NULL	factor Xa	GP		bind		cooperatively			EPR-1	GP	vascular cell			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_13_8340_s_150	9079657	2 Altogether, these data suggest a cooperative model of factor Xa binding to vascular cell EPR-1, potentially involving an initial Gla-dependent contact stabilized by an high affinity recognition of the inter-EGF sequence 83-88, and followed by an as yet unidentified step of local proteolysis by cell surface-bound factor Xa for downstream signal transduction events and effector responses ( 19).	bind
28379	2	6948	5	13	NULL	NULL	NULL	statement 1	Process		involve		potentially			Gla-dependent contact	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_13_8340_s_150	9079657	2 Altogether, these data suggest a cooperative model of factor Xa binding to vascular cell EPR-1, potentially involving an initial Gla-dependent contact stabilized by an high affinity recognition of the inter-EGF sequence 83-88, and followed by an as yet unidentified step of local proteolysis by cell surface-bound factor Xa for downstream signal transduction events and effector responses ( 19).	bind
28380	3	6948	5	13	NULL	NULL	NULL	Gla-dependent contact	Process		is stabilized by							high affinity recognition of	inter-EGF sequence		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_13_8340_s_150	9079657	2 Altogether, these data suggest a cooperative model of factor Xa binding to vascular cell EPR-1, potentially involving an initial Gla-dependent contact stabilized by an high affinity recognition of the inter-EGF sequence 83-88, and followed by an as yet unidentified step of local proteolysis by cell surface-bound factor Xa for downstream signal transduction events and effector responses ( 19).	bind
28381	4	6948	5	13	NULL	NULL	NULL	statement 2	Process		is followed by					local proteolysis	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_13_8340_s_150	9079657	2 Altogether, these data suggest a cooperative model of factor Xa binding to vascular cell EPR-1, potentially involving an initial Gla-dependent contact stabilized by an high affinity recognition of the inter-EGF sequence 83-88, and followed by an as yet unidentified step of local proteolysis by cell surface-bound factor Xa for downstream signal transduction events and effector responses ( 19).	bind
28383	6	6948	5	13	NULL	NULL	NULL	statement 5	Process		is required for					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_13_8340_s_150	9079657	2 Altogether, these data suggest a cooperative model of factor Xa binding to vascular cell EPR-1, potentially involving an initial Gla-dependent contact stabilized by an high affinity recognition of the inter-EGF sequence 83-88, and followed by an as yet unidentified step of local proteolysis by cell surface-bound factor Xa for downstream signal transduction events and effector responses ( 19).	bind
28391	7	6948	5	13	NULL	NULL	NULL	statement 4	Process		leads to					signal transduction events	Process	downstream			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_13_8340_s_150	9079657	2 Altogether, these data suggest a cooperative model of factor Xa binding to vascular cell EPR-1, potentially involving an initial Gla-dependent contact stabilized by an high affinity recognition of the inter-EGF sequence 83-88, and followed by an as yet unidentified step of local proteolysis by cell surface-bound factor Xa for downstream signal transduction events and effector responses ( 19).	bind
28394	8	6948	5	13	NULL	NULL	NULL	statement 4	Process		leads to					effector responses	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_13_8340_s_150	9079657	2 Altogether, these data suggest a cooperative model of factor Xa binding to vascular cell EPR-1, potentially involving an initial Gla-dependent contact stabilized by an high affinity recognition of the inter-EGF sequence 83-88, and followed by an as yet unidentified step of local proteolysis by cell surface-bound factor Xa for downstream signal transduction events and effector responses ( 19).	bind
44797	5	6948	5	13	NULL	NULL	NULL	factor Xa	GP		bind					cell surface	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_13_8340_s_150	9079657	2 Altogether, these data suggest a cooperative model of factor Xa binding to vascular cell EPR-1, potentially involving an initial Gla-dependent contact stabilized by an high affinity recognition of the inter-EGF sequence 83-88, and followed by an as yet unidentified step of local proteolysis by cell surface-bound factor Xa for downstream signal transduction events and effector responses ( 19).	bind
20787	1	6948	6	13	NULL	NULL	NULL	factor Xa	GP		bind					EPR-1	GP	vascular cell			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_13_8340_s_150	9079657	2 Altogether, these data suggest a cooperative model of factor Xa binding to vascular cell EPR-1, potentially involving an initial Gla-dependent contact stabilized by an high affinity recognition of the inter-EGF sequence 83-88, and followed by an as yet unidentified step of local proteolysis by cell surface-bound factor Xa for downstream signal transduction events and effector responses ( 19).	bind
21185	5	6948	6	10	NULL	0	NULL	statement 3			followed by					local proteolysis					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_13_8340_s_150	9079657	2 Altogether, these data suggest a cooperative model of factor Xa binding to vascular cell EPR-1, potentially involving an initial Gla-dependent contact stabilized by an high affinity recognition of the inter-EGF sequence 83-88, and followed by an as yet unidentified step of local proteolysis by cell surface-bound factor Xa for downstream signal transduction events and effector responses ( 19).	bind
21551	3	6948	6	NULL	NULL	0	NULL	Gla dependent contact	NULL		is involved in	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_13_8340_s_150	9079657	2 Altogether, these data suggest a cooperative model of factor Xa binding to vascular cell EPR-1, potentially involving an initial Gla-dependent contact stabilized by an high affinity recognition of the inter-EGF sequence 83-88, and followed by an as yet unidentified step of local proteolysis by cell surface-bound factor Xa for downstream signal transduction events and effector responses ( 19).	bind
21552	4	6948	6	10	NULL	0	NULL	statement 3			is stabilized by							high affinity recognition of	inter-EGF sequence 83-88		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_13_8340_s_150	9079657	2 Altogether, these data suggest a cooperative model of factor Xa binding to vascular cell EPR-1, potentially involving an initial Gla-dependent contact stabilized by an high affinity recognition of the inter-EGF sequence 83-88, and followed by an as yet unidentified step of local proteolysis by cell surface-bound factor Xa for downstream signal transduction events and effector responses ( 19).	bind
21553	6	6948	6	10	NULL	0	NULL	statement 2			is required for					statement 5					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_13_8340_s_150	9079657	2 Altogether, these data suggest a cooperative model of factor Xa binding to vascular cell EPR-1, potentially involving an initial Gla-dependent contact stabilized by an high affinity recognition of the inter-EGF sequence 83-88, and followed by an as yet unidentified step of local proteolysis by cell surface-bound factor Xa for downstream signal transduction events and effector responses ( 19).	bind
44798	2	6948	6	10	NULL	0	NULL	factor Xa	NULL		bind	NULL				cell surface	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_13_8340_s_150	9079657	2 Altogether, these data suggest a cooperative model of factor Xa binding to vascular cell EPR-1, potentially involving an initial Gla-dependent contact stabilized by an high affinity recognition of the inter-EGF sequence 83-88, and followed by an as yet unidentified step of local proteolysis by cell surface-bound factor Xa for downstream signal transduction events and effector responses ( 19).	bind
56790	7	6948	6	10	NULL	0	NULL	statement 5			lead to					signal transduction events		downstream			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_13_8340_s_150	9079657	2 Altogether, these data suggest a cooperative model of factor Xa binding to vascular cell EPR-1, potentially involving an initial Gla-dependent contact stabilized by an high affinity recognition of the inter-EGF sequence 83-88, and followed by an as yet unidentified step of local proteolysis by cell surface-bound factor Xa for downstream signal transduction events and effector responses ( 19).	bind
56791	8	6948	6	10	NULL	0	NULL	statement 5			lead to					effector responses					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_13_8340_s_150	9079657	2 Altogether, these data suggest a cooperative model of factor Xa binding to vascular cell EPR-1, potentially involving an initial Gla-dependent contact stabilized by an high affinity recognition of the inter-EGF sequence 83-88, and followed by an as yet unidentified step of local proteolysis by cell surface-bound factor Xa for downstream signal transduction events and effector responses ( 19).	bind
25215	1	6949	5	13	NULL	NULL	NULL	Gal80p	GP		undergoes					dimerization	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13485_s_20	16524886	2 An inhibitory protein Gal80p dimerizes and binds to nuclear Gal4p in the absence of galactose, preventing recruitment of activator proteins by Gal4p and effectively repressing gene expression.	bind
25216	2	6949	5	13	NULL	NULL	NULL	statement 1	GP		bind					Gal4p	GP	nuclear			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13485_s_20	16524886	2 An inhibitory protein Gal80p dimerizes and binds to nuclear Gal4p in the absence of galactose, preventing recruitment of activator proteins by Gal4p and effectively repressing gene expression.	bind
25217	3	6949	5	13	NULL	NULL	NULL	statement 2	Process		in the absence of					galactose	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13485_s_20	16524886	2 An inhibitory protein Gal80p dimerizes and binds to nuclear Gal4p in the absence of galactose, preventing recruitment of activator proteins by Gal4p and effectively repressing gene expression.	bind
25218	4	6949	5	13	NULL	NULL	NULL	Gal4p	GP		recruits					activator proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13485_s_20	16524886	2 An inhibitory protein Gal80p dimerizes and binds to nuclear Gal4p in the absence of galactose, preventing recruitment of activator proteins by Gal4p and effectively repressing gene expression.	bind
25219	5	6949	5	13	NULL	NULL	NULL	statement 3	Process		prevents					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13485_s_20	16524886	2 An inhibitory protein Gal80p dimerizes and binds to nuclear Gal4p in the absence of galactose, preventing recruitment of activator proteins by Gal4p and effectively repressing gene expression.	bind
25220	6	6949	5	13	NULL	NULL	NULL	statement 3	Process		represses		effectively			gene expression	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13485_s_20	16524886	2 An inhibitory protein Gal80p dimerizes and binds to nuclear Gal4p in the absence of galactose, preventing recruitment of activator proteins by Gal4p and effectively repressing gene expression.	bind
44799	7	6949	5	13	NULL	NULL	NULL	Gal80p	GP		is a type of					inhibitory protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13485_s_20	16524886	2 An inhibitory protein Gal80p dimerizes and binds to nuclear Gal4p in the absence of galactose, preventing recruitment of activator proteins by Gal4p and effectively repressing gene expression.	bind
20789	2	6949	6	10	NULL	0	NULL	statement 1			bind					Gal4p		nuclear			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13485_s_20	16524886	2 An inhibitory protein Gal80p dimerizes and binds to nuclear Gal4p in the absence of galactose, preventing recruitment of activator proteins by Gal4p and effectively repressing gene expression.	bind
20911	1	6949	6	10	NULL	0	NULL	Gal80p			bind					Gal80p					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13485_s_20	16524886	2 An inhibitory protein Gal80p dimerizes and binds to nuclear Gal4p in the absence of galactose, preventing recruitment of activator proteins by Gal4p and effectively repressing gene expression.	bind
20912	3	6949	6	10	NULL	0	NULL	statement 2			occurs in absence of					galactose					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13485_s_20	16524886	2 An inhibitory protein Gal80p dimerizes and binds to nuclear Gal4p in the absence of galactose, preventing recruitment of activator proteins by Gal4p and effectively repressing gene expression.	bind
20914	4	6949	6	10	NULL	0	NULL	Gal4p			recruits					activator proteins					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13485_s_20	16524886	2 An inhibitory protein Gal80p dimerizes and binds to nuclear Gal4p in the absence of galactose, preventing recruitment of activator proteins by Gal4p and effectively repressing gene expression.	bind
20916	5	6949	6	10	NULL	0	NULL	statement 2			prevents					statement 4					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13485_s_20	16524886	2 An inhibitory protein Gal80p dimerizes and binds to nuclear Gal4p in the absence of galactose, preventing recruitment of activator proteins by Gal4p and effectively repressing gene expression.	bind
20924	6	6949	6	10	NULL	0	NULL	statement 2			repress		effectively			gene expression					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13485_s_20	16524886	2 An inhibitory protein Gal80p dimerizes and binds to nuclear Gal4p in the absence of galactose, preventing recruitment of activator proteins by Gal4p and effectively repressing gene expression.	bind
44800	7	6949	6	10	NULL	0	NULL	Ga180p			is a type of					inhibitory protein					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13485_s_20	16524886	2 An inhibitory protein Gal80p dimerizes and binds to nuclear Gal4p in the absence of galactose, preventing recruitment of activator proteins by Gal4p and effectively repressing gene expression.	bind
25221	1	6950	5	13	NULL	NULL	NULL	Grb2	GP		bind					TrkA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_24_18225_s_134	10748052	2 and  19) providing further evidence that Grb2 binds to TrkA independently of Shc/FRS-2.	bind
25222	2	6950	5	13	NULL	NULL	NULL	statement 1	Process		is independent of					Shc/FRS-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_24_18225_s_134	10748052	2 and  19) providing further evidence that Grb2 binds to TrkA independently of Shc/FRS-2.	bind
20928	1	6950	6	NULL	NULL	0	NULL	Grb2	NULL		bind	NULL				TrkA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_24_18225_s_134	10748052	2 and  19) providing further evidence that Grb2 binds to TrkA independently of Shc/FRS-2.	bind
20929	2	6950	6	NULL	NULL	0	NULL	statement 1	NULL		is independent of	NULL				Shc/FRS-2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_24_18225_s_134	10748052	2 and  19) providing further evidence that Grb2 binds to TrkA independently of Shc/FRS-2.	bind
25226	1	6952	5	13	NULL	NULL	NULL	octasccharides	Chemical	3H- labeled	bind					FGF-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_33_30744_s_90	11406624	2 Approximately 25% of the 3H-labeled octasaccharides derived from intestinal HS bound to the FGF-1 column at physiological ionic strength.	bind
31491	2	6952	5	13	NULL	NULL	NULL	octasaccharides	Chemical	3H-labeled	derived from					HS	Chemical	intestinal			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_33_30744_s_90	11406624	2 Approximately 25% of the 3H-labeled octasaccharides derived from intestinal HS bound to the FGF-1 column at physiological ionic strength.	bind
31492	3	6952	5	13	NULL	NULL	NULL	statement 1	Process		occurs at					physiological ionic strength	QuantityOrMeasure				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_33_30744_s_90	11406624	2 Approximately 25% of the 3H-labeled octasaccharides derived from intestinal HS bound to the FGF-1 column at physiological ionic strength.	bind
20932	1	6952	6	10	NULL	0	NULL	octasaccharides		3H-labeled	derived from					 HS		intestinal			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_33_30744_s_90	11406624	2 Approximately 25% of the 3H-labeled octasaccharides derived from intestinal HS bound to the FGF-1 column at physiological ionic strength.	bind
20933	2	6952	6	NULL	NULL	0	NULL	octasaccharides	NULL	3H-labeled	bind	NULL				FGF-1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_33_30744_s_90	11406624	2 Approximately 25% of the 3H-labeled octasaccharides derived from intestinal HS bound to the FGF-1 column at physiological ionic strength.	bind
20947	3	6952	6	10	NULL	0	NULL	statement 2			occurs at					physiological ionic strength					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_33_30744_s_90	11406624	2 Approximately 25% of the 3H-labeled octasaccharides derived from intestinal HS bound to the FGF-1 column at physiological ionic strength.	bind
25227	1	6954	5	13	NULL	NULL	NULL	GST-GRK5 	GP		bind			1-200		calmodulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_29_18273_s_203	9218466	2 As expected, the 1-200- and 20-39-containing GST-GRK5 fusion proteins bound to calmodulin, whereas the 98-136 and 50-200 fusions did not.	bind
31496	2	6954	5	13	NULL	NULL	NULL	GST-GRK5 	GP		bind			20-39		calmodulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_29_18273_s_203	9218466	2 As expected, the 1-200- and 20-39-containing GST-GRK5 fusion proteins bound to calmodulin, whereas the 98-136 and 50-200 fusions did not.	bind
31497	3	6954	5	13	NULL	NULL	NULL	GST-GRK5 	GP		does not bind			98-136		calmodulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_29_18273_s_203	9218466	2 As expected, the 1-200- and 20-39-containing GST-GRK5 fusion proteins bound to calmodulin, whereas the 98-136 and 50-200 fusions did not.	bind
31499	4	6954	5	13	NULL	NULL	NULL	GST-GRK5 	GP		does not bind			50-200		calmodulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_29_18273_s_203	9218466	2 As expected, the 1-200- and 20-39-containing GST-GRK5 fusion proteins bound to calmodulin, whereas the 98-136 and 50-200 fusions did not.	bind
44801	5	6954	5	13	NULL	NULL	NULL	GST-GRK5	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_29_18273_s_203	9218466	2 As expected, the 1-200- and 20-39-containing GST-GRK5 fusion proteins bound to calmodulin, whereas the 98-136 and 50-200 fusions did not.	bind
20948	1	6954	6	10	NULL	0	NULL	GST-GRK5 	NULL		bind	NULL		1-200		calmodulin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_29_18273_s_203	9218466	2 As expected, the 1-200- and 20-39-containing GST-GRK5 fusion proteins bound to calmodulin, whereas the 98-136 and 50-200 fusions did not.	bind
20949	2	6954	6	10	NULL	0	NULL	GST-GRK5	NULL		bind	NULL		20-39		calmodulin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_29_18273_s_203	9218466	2 As expected, the 1-200- and 20-39-containing GST-GRK5 fusion proteins bound to calmodulin, whereas the 98-136 and 50-200 fusions did not.	bind
20950	3	6954	6	10	NULL	0	NULL	GST-GRK5	NULL		does not bind	NULL		98-136		calmodulin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_29_18273_s_203	9218466	2 As expected, the 1-200- and 20-39-containing GST-GRK5 fusion proteins bound to calmodulin, whereas the 98-136 and 50-200 fusions did not.	bind
20951	4	6954	6	10	NULL	0	NULL	GST-GRK5 	NULL		does not bind	NULL		50-200		calmodulin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_29_18273_s_203	9218466	2 As expected, the 1-200- and 20-39-containing GST-GRK5 fusion proteins bound to calmodulin, whereas the 98-136 and 50-200 fusions did not.	bind
44802	5	6954	6	10	NULL	0	NULL	GST-GRK5	NULL		is a type of	NULL				fusion protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_29_18273_s_203	9218466	2 As expected, the 1-200- and 20-39-containing GST-GRK5 fusion proteins bound to calmodulin, whereas the 98-136 and 50-200 fusions did not.	bind
25228	1	6955	5	13	NULL	NULL	NULL	Vps21p	GP		bind			S21N		GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_15284_s_126	10329739	2 As shown in Fig.  1 B, Vps21p-S21N bound substantially more GDP (26 pmol) than GTP (<2 pmol).	bind
25229	2	6955	5	13	NULL	NULL	NULL	Vps21p	GP		bind			S21N		GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_15284_s_126	10329739	2 As shown in Fig.  1 B, Vps21p-S21N bound substantially more GDP (26 pmol) than GTP (<2 pmol).	bind
25230	3	6955	5	13	NULL	NULL	NULL	statement 1	Process		more than		substantially			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_15284_s_126	10329739	2 As shown in Fig.  1 B, Vps21p-S21N bound substantially more GDP (26 pmol) than GTP (<2 pmol).	bind
20952	1	6955	6	NULL	NULL	0	NULL	Vps21p	NULL		bind	NULL		S21N		GDP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_21_15284_s_126	10329739	2 As shown in Fig.  1 B, Vps21p-S21N bound substantially more GDP (26 pmol) than GTP (<2 pmol).	bind
20953	2	6955	6	NULL	NULL	0	NULL	Vps21p	NULL		bind	NULL		S21N		GTP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_21_15284_s_126	10329739	2 As shown in Fig.  1 B, Vps21p-S21N bound substantially more GDP (26 pmol) than GTP (<2 pmol).	bind
20954	3	6955	6	10	NULL	0	NULL	statement 1			is more than		substantially			statement 2					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_15284_s_126	10329739	2 As shown in Fig.  1 B, Vps21p-S21N bound substantially more GDP (26 pmol) than GTP (<2 pmol).	bind
25231	1	6956	5	13	NULL	NULL	NULL	TGF-beta1	GP		bind					TbetaRII	GP	soluble			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_48_30656_s_87	8940041	2 As shown in Fig.  1, TGF-beta1 binds soluble TbetaRII at all of the different coating concentrations, whereas under the same conditions, the binding of TGF-beta2 is detectable only at the highest coating concentration of TbetaRII (100 ng/well).	bind
25232	2	6956	5	13	NULL	NULL	NULL	TGF-beta2	GP		bind					TbetaRII	GP	soluble			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_48_30656_s_87	8940041	2 As shown in Fig.  1, TGF-beta1 binds soluble TbetaRII at all of the different coating concentrations, whereas under the same conditions, the binding of TGF-beta2 is detectable only at the highest coating concentration of TbetaRII (100 ng/well).	bind
20955	1	6956	6	NULL	NULL	0	NULL	TGF-beta1	NULL		bind	NULL				TbetaRII	NULL	soluble			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_48_30656_s_87	8940041	2 As shown in Fig.  1, TGF-beta1 binds soluble TbetaRII at all of the different coating concentrations, whereas under the same conditions, the binding of TGF-beta2 is detectable only at the highest coating concentration of TbetaRII (100 ng/well).	bind
30685	2	6956	6	NULL	NULL	0	NULL	TGF-beta2	NULL		bind	NULL				TbetaRII	NULL	soluble			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_48_30656_s_87	8940041	2 As shown in Fig.  1, TGF-beta1 binds soluble TbetaRII at all of the different coating concentrations, whereas under the same conditions, the binding of TGF-beta2 is detectable only at the highest coating concentration of TbetaRII (100 ng/well).	bind
25234	1	6957	5	13	NULL	NULL	NULL	Csk	GP	purified	bind					Syk	GP	endogenous			NULL	DT40 whole-cell extracts	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_27_17209_s_158	9202044	2 As shown in Fig.  5 B, purified Csk, Lyn, and Btk bound to the endogenous Syk from the DT40 whole-cell extracts, while a control His6-tagged protein (NF-AT-His6, a T-cell-specific transcription factor) did not.	bind
25235	2	6957	5	13	NULL	NULL	NULL	Lyn	GP	purified	bind					Syk	GP	endogenous			NULL	DT40 whole-cell extracts	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_27_17209_s_158	9202044	2 As shown in Fig.  5 B, purified Csk, Lyn, and Btk bound to the endogenous Syk from the DT40 whole-cell extracts, while a control His6-tagged protein (NF-AT-His6, a T-cell-specific transcription factor) did not.	bind
25236	3	6957	5	13	NULL	NULL	NULL	Btk	GP	purified	bind					Syk	GP	endogenous			NULL	DT40 whole-cell extracts	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_27_17209_s_158	9202044	2 As shown in Fig.  5 B, purified Csk, Lyn, and Btk bound to the endogenous Syk from the DT40 whole-cell extracts, while a control His6-tagged protein (NF-AT-His6, a T-cell-specific transcription factor) did not.	bind
25237	4	6957	5	13	NULL	NULL	NULL	NF-AT-His6	GP		does not bind					Syk	GP	endogenous			NULL	DT40 whole-cell extracts	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_27_17209_s_158	9202044	2 As shown in Fig.  5 B, purified Csk, Lyn, and Btk bound to the endogenous Syk from the DT40 whole-cell extracts, while a control His6-tagged protein (NF-AT-His6, a T-cell-specific transcription factor) did not.	bind
31501	5	6957	5	13	NULL	NULL	NULL	NF-AT-His6	GP		is a type of					T-cell-specific transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_27_17209_s_158	9202044	2 As shown in Fig.  5 B, purified Csk, Lyn, and Btk bound to the endogenous Syk from the DT40 whole-cell extracts, while a control His6-tagged protein (NF-AT-His6, a T-cell-specific transcription factor) did not.	bind
20956	1	6957	6	NULL	NULL	0	NULL	Csk	NULL	purified	bind	NULL				Syk	NULL	endogenous			NULL	DT40 whole-cell extracts	0	NULL	NULL	NULL	gw60_jbiolchem_272_27_17209_s_158	9202044	2 As shown in Fig.  5 B, purified Csk, Lyn, and Btk bound to the endogenous Syk from the DT40 whole-cell extracts, while a control His6-tagged protein (NF-AT-His6, a T-cell-specific transcription factor) did not.	bind
20957	2	6957	6	NULL	NULL	0	NULL	Lyn	NULL	purified	bind	NULL				Syk	NULL	endogenous			NULL	DT40 whole-cell extracts	0	NULL	NULL	NULL	gw60_jbiolchem_272_27_17209_s_158	9202044	2 As shown in Fig.  5 B, purified Csk, Lyn, and Btk bound to the endogenous Syk from the DT40 whole-cell extracts, while a control His6-tagged protein (NF-AT-His6, a T-cell-specific transcription factor) did not.	bind
20958	3	6957	6	NULL	NULL	0	NULL	Btk	NULL	purified	bind	NULL				Syk	NULL	endogenous			NULL	DT40 whole-cell extracts	0	NULL	NULL	NULL	gw60_jbiolchem_272_27_17209_s_158	9202044	2 As shown in Fig.  5 B, purified Csk, Lyn, and Btk bound to the endogenous Syk from the DT40 whole-cell extracts, while a control His6-tagged protein (NF-AT-His6, a T-cell-specific transcription factor) did not.	bind
20959	4	6957	6	NULL	NULL	0	NULL	NF-AT-His6	NULL		is a type of	NULL				T-cell-specific transcription factor	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_27_17209_s_158	9202044	2 As shown in Fig.  5 B, purified Csk, Lyn, and Btk bound to the endogenous Syk from the DT40 whole-cell extracts, while a control His6-tagged protein (NF-AT-His6, a T-cell-specific transcription factor) did not.	bind
20960	5	6957	6	NULL	NULL	0	NULL	NF-AT-His6	NULL		does not bind	NULL				Syk	NULL	endogenous			NULL	DT40 whole-cell extracts	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_27_17209_s_158	9202044	2 As shown in Fig.  5 B, purified Csk, Lyn, and Btk bound to the endogenous Syk from the DT40 whole-cell extracts, while a control His6-tagged protein (NF-AT-His6, a T-cell-specific transcription factor) did not.	bind
25238	1	6958	5	13	NULL	NULL	NULL	Rab7	GP		bind					REP-1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_52_48637_s_224	11675392	2 At low concentrations of components, when the dissociation rates govern the kinetics, binding of Rab7 to REP-1 and the second prenylation step would become rate-limiting (Scheme  1).	bind
20961	1	6958	6	NULL	NULL	0	NULL	Rab7	NULL		bind	NULL				REP-1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_52_48637_s_224	11675392	2 At low concentrations of components, when the dissociation rates govern the kinetics, binding of Rab7 to REP-1 and the second prenylation step would become rate-limiting (Scheme  1).	bind
25241	1	6959	5	13	NULL	NULL	NULL	hRAD51 NPF	GP		bind					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_29_30385_s_298	15123651	2 Based on its ADP ATP exchange activity, these observations suggest that hXRCC2 promotes the ATP-bound form of the hRAD51 NPF.	bind
25242	2	6959	5	13	NULL	NULL	NULL	hXRCC2	GP		promotes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_29_30385_s_298	15123651	2 Based on its ADP ATP exchange activity, these observations suggest that hXRCC2 promotes the ATP-bound form of the hRAD51 NPF.	bind
20962	1	6959	6	NULL	NULL	0	NULL	hRAD51 NPF	NULL		bind	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_29_30385_s_298	15123651	2 Based on its ADP ATP exchange activity, these observations suggest that hXRCC2 promotes the ATP-bound form of the hRAD51 NPF.	bind
20963	2	6959	6	NULL	NULL	0	NULL	hXRCC2	NULL		promotes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_29_30385_s_298	15123651	2 Based on its ADP ATP exchange activity, these observations suggest that hXRCC2 promotes the ATP-bound form of the hRAD51 NPF.	bind
25243	1	6960	5	13	NULL	NULL	NULL	eIF4E	GP	mutations in	effects		differentially			eIF4G	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_30_21297_s_27	10409688	2 Based on the findings that mutations in eIF4E have differential effects on the binding of eIF4G and Caf20p, it has been suggested that the interactions of eIF4G and the 4E-BPs with eIF4E are not limited to the eIF4E binding peptide ( 19).	bind
25244	2	6960	5	13	NULL	NULL	NULL	eIF4E	GP	mutations in	effects		differentially			Caf20p	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_30_21297_s_27	10409688	2 Based on the findings that mutations in eIF4E have differential effects on the binding of eIF4G and Caf20p, it has been suggested that the interactions of eIF4G and the 4E-BPs with eIF4E are not limited to the eIF4E binding peptide ( 19).	bind
25245	3	6960	5	13	NULL	NULL	NULL	eIF4G	GP		interacts with					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_30_21297_s_27	10409688	2 Based on the findings that mutations in eIF4E have differential effects on the binding of eIF4G and Caf20p, it has been suggested that the interactions of eIF4G and the 4E-BPs with eIF4E are not limited to the eIF4E binding peptide ( 19).	bind
25246	4	6960	5	13	NULL	NULL	NULL	statement 3	Process		is not limited to					eIF4E binding peptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_30_21297_s_27	10409688	2 Based on the findings that mutations in eIF4E have differential effects on the binding of eIF4G and Caf20p, it has been suggested that the interactions of eIF4G and the 4E-BPs with eIF4E are not limited to the eIF4E binding peptide ( 19).	bind
25247	5	6960	5	13	NULL	NULL	NULL	4E-BPs	GP		interacts with					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_30_21297_s_27	10409688	2 Based on the findings that mutations in eIF4E have differential effects on the binding of eIF4G and Caf20p, it has been suggested that the interactions of eIF4G and the 4E-BPs with eIF4E are not limited to the eIF4E binding peptide ( 19).	bind
25248	6	6960	5	13	NULL	NULL	NULL	statement 5	Process		is not limited to					eIF4E binding peptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_30_21297_s_27	10409688	2 Based on the findings that mutations in eIF4E have differential effects on the binding of eIF4G and Caf20p, it has been suggested that the interactions of eIF4G and the 4E-BPs with eIF4E are not limited to the eIF4E binding peptide ( 19).	bind
20965	1	6960	6	10	NULL	0	NULL	eIF4E		mutations in	effects		differentially			eIF4G		binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_30_21297_s_27	10409688	2 Based on the findings that mutations in eIF4E have differential effects on the binding of eIF4G and Caf20p, it has been suggested that the interactions of eIF4G and the 4E-BPs with eIF4E are not limited to the eIF4E binding peptide ( 19).	bind
20966	2	6960	6	10	NULL	0	NULL	eIF4E		mutations in	effect		differentially			Caf20p		binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_30_21297_s_27	10409688	2 Based on the findings that mutations in eIF4E have differential effects on the binding of eIF4G and Caf20p, it has been suggested that the interactions of eIF4G and the 4E-BPs with eIF4E are not limited to the eIF4E binding peptide ( 19).	bind
20967	3	6960	6	NULL	NULL	0	NULL	eIF4G	NULL		interacts with	NULL				eIF4E	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21297_s_27	10409688	2 Based on the findings that mutations in eIF4E have differential effects on the binding of eIF4G and Caf20p, it has been suggested that the interactions of eIF4G and the 4E-BPs with eIF4E are not limited to the eIF4E binding peptide ( 19).	bind
20968	4	6960	6	NULL	NULL	0	NULL	4E-BP	NULL		interacts with	NULL				eIF4E	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21297_s_27	10409688	2 Based on the findings that mutations in eIF4E have differential effects on the binding of eIF4G and Caf20p, it has been suggested that the interactions of eIF4G and the 4E-BPs with eIF4E are not limited to the eIF4E binding peptide ( 19).	bind
20969	5	6960	6	NULL	NULL	0	NULL	statement 3	NULL		is not limited to	NULL				eIF4E binding peptide	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21297_s_27	10409688	2 Based on the findings that mutations in eIF4E have differential effects on the binding of eIF4G and Caf20p, it has been suggested that the interactions of eIF4G and the 4E-BPs with eIF4E are not limited to the eIF4E binding peptide ( 19).	bind
20970	6	6960	6	NULL	NULL	0	NULL	statement 4	NULL		is not limited to	NULL				eIF4E binding peptide	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21297_s_27	10409688	2 Based on the findings that mutations in eIF4E have differential effects on the binding of eIF4G and Caf20p, it has been suggested that the interactions of eIF4G and the 4E-BPs with eIF4E are not limited to the eIF4E binding peptide ( 19).	bind
25249	1	6961	5	13	NULL	NULL	NULL	Rtg2p	GP		does not bind					Rtg1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_19801_s_159	9242640	2 Based on two-hybrid analysis carried out in the current study, we conclude that Rtg2p neither binds to Rtg1p or Rtg3p nor is required for the  direct interaction of these transcription factors with each other.	bind
25250	2	6961	5	13	NULL	NULL	NULL	Rtg2p	GP		does not bind					Rtg3p	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_19801_s_159	9242640	2 Based on two-hybrid analysis carried out in the current study, we conclude that Rtg2p neither binds to Rtg1p or Rtg3p nor is required for the  direct interaction of these transcription factors with each other.	bind
25252	3	6961	5	13	NULL	NULL	NULL	Rtg1p	GP		interacts with		directly			Rtg3p	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_19801_s_159	9242640	2 Based on two-hybrid analysis carried out in the current study, we conclude that Rtg2p neither binds to Rtg1p or Rtg3p nor is required for the  direct interaction of these transcription factors with each other.	bind
25253	4	6961	5	13	NULL	NULL	NULL	Rtg2p	GP		is not required for					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_19801_s_159	9242640	2 Based on two-hybrid analysis carried out in the current study, we conclude that Rtg2p neither binds to Rtg1p or Rtg3p nor is required for the  direct interaction of these transcription factors with each other.	bind
31506	5	6961	5	13	NULL	NULL	NULL	Rtg2p	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_19801_s_159	9242640	2 Based on two-hybrid analysis carried out in the current study, we conclude that Rtg2p neither binds to Rtg1p or Rtg3p nor is required for the  direct interaction of these transcription factors with each other.	bind
31507	6	6961	5	13	NULL	NULL	NULL	Rtg1p	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_19801_s_159	9242640	2 Based on two-hybrid analysis carried out in the current study, we conclude that Rtg2p neither binds to Rtg1p or Rtg3p nor is required for the  direct interaction of these transcription factors with each other.	bind
31508	7	6961	5	13	NULL	NULL	NULL	Rtg3p	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_19801_s_159	9242640	2 Based on two-hybrid analysis carried out in the current study, we conclude that Rtg2p neither binds to Rtg1p or Rtg3p nor is required for the  direct interaction of these transcription factors with each other.	bind
20971	1	6961	6	NULL	NULL	0	NULL	Rtg2p	NULL		does not bind	NULL				Rtg1p	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_32_19801_s_159	9242640	2 Based on two-hybrid analysis carried out in the current study, we conclude that Rtg2p neither binds to Rtg1p or Rtg3p nor is required for the  direct interaction of these transcription factors with each other.	bind
20972	2	6961	6	NULL	NULL	0	NULL	Rtg2p	NULL		does not bind	NULL				Rtg3p	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_32_19801_s_159	9242640	2 Based on two-hybrid analysis carried out in the current study, we conclude that Rtg2p neither binds to Rtg1p or Rtg3p nor is required for the  direct interaction of these transcription factors with each other.	bind
20973	3	6961	6	NULL	NULL	0	NULL	Rtg1p 	NULL		interacts with	NULL	directly			Rtg3p	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_19801_s_159	9242640	2 Based on two-hybrid analysis carried out in the current study, we conclude that Rtg2p neither binds to Rtg1p or Rtg3p nor is required for the  direct interaction of these transcription factors with each other.	bind
20974	4	6961	6	NULL	NULL	0	NULL	Rtg2p	NULL		is not required for	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_32_19801_s_159	9242640	2 Based on two-hybrid analysis carried out in the current study, we conclude that Rtg2p neither binds to Rtg1p or Rtg3p nor is required for the  direct interaction of these transcription factors with each other.	bind
30686	5	6961	6	NULL	NULL	0	NULL	Rtg1p	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_32_19801_s_159	9242640	2 Based on two-hybrid analysis carried out in the current study, we conclude that Rtg2p neither binds to Rtg1p or Rtg3p nor is required for the  direct interaction of these transcription factors with each other.	bind
30687	6	6961	6	NULL	NULL	0	NULL	Rtg2p	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_32_19801_s_159	9242640	2 Based on two-hybrid analysis carried out in the current study, we conclude that Rtg2p neither binds to Rtg1p or Rtg3p nor is required for the  direct interaction of these transcription factors with each other.	bind
30688	7	6961	6	NULL	NULL	0	NULL	Rtg3p	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_32_19801_s_159	9242640	2 Based on two-hybrid analysis carried out in the current study, we conclude that Rtg2p neither binds to Rtg1p or Rtg3p nor is required for the  direct interaction of these transcription factors with each other.	bind
25254	1	6962	5	13	NULL	NULL	NULL	DnaB	GP		bind		stably			prepriming complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34255_s_207	9852089	2 Because a similar mechanism is likely to occur at  oriC, we conclude that the defect of the N-terminal deletions in Form 1* formation is in promoting the stable binding of DnaB to the prepriming complex.	bind
31509	2	6962	5	13	NULL	NULL	NULL	Form 1* formation	Process		promote			N-terminal deletion defects		statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34255_s_207	9852089	2 Because a similar mechanism is likely to occur at  oriC, we conclude that the defect of the N-terminal deletions in Form 1* formation is in promoting the stable binding of DnaB to the prepriming complex.	bind
20975	1	6962	6	10	NULL	0	NULL	DnaB			bind		stably			prepriming complex					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34255_s_207	9852089	2 Because a similar mechanism is likely to occur at  oriC, we conclude that the defect of the N-terminal deletions in Form 1* formation is in promoting the stable binding of DnaB to the prepriming complex.	bind
21186	2	6962	6	10	NULL	0	NULL	Form 1* formation	NULL		promotes	NULL		N-terminal deletion defects		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34255_s_207	9852089	2 Because a similar mechanism is likely to occur at  oriC, we conclude that the defect of the N-terminal deletions in Form 1* formation is in promoting the stable binding of DnaB to the prepriming complex.	bind
25255	1	6963	5	13	NULL	NULL	NULL	eRF3	GP		interacts with					PAN deadenylase	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45693_s_312	15337765	2 Because eRF3 interacts with PAN deadenylase, the GDP-bound form of eRF3 might recruit PAN after translation termination to mediate poly	bind
25256	3	6963	5	13	NULL	NULL	NULL	statement 2	GP		recruits		might			PAN	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45693_s_312	15337765	2 Because eRF3 interacts with PAN deadenylase, the GDP-bound form of eRF3 might recruit PAN after translation termination to mediate poly	bind
25257	4	6963	5	13	NULL	NULL	NULL	statement 3	Process		occurs after					translation	Process	termination of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45693_s_312	15337765	2 Because eRF3 interacts with PAN deadenylase, the GDP-bound form of eRF3 might recruit PAN after translation termination to mediate poly	bind
31510	2	6963	5	13	NULL	NULL	NULL	eRF3	GP		bind					GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_44_45693_s_312	15337765	2 Because eRF3 interacts with PAN deadenylase, the GDP-bound form of eRF3 might recruit PAN after translation termination to mediate poly	bind
20976	1	6963	6	NULL	NULL	0	NULL	eRF3	NULL		interacts with	NULL				PAN deadenylase	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_44_45693_s_312	15337765	2 Because eRF3 interacts with PAN deadenylase, the GDP-bound form of eRF3 might recruit PAN after translation termination to mediate poly	bind
20977	2	6963	6	NULL	NULL	0	NULL	eRF3	NULL		bind	NULL				GDP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_44_45693_s_312	15337765	2 Because eRF3 interacts with PAN deadenylase, the GDP-bound form of eRF3 might recruit PAN after translation termination to mediate poly	bind
20978	3	6963	6	NULL	NULL	0	NULL	statement 2	NULL		recruit	NULL	might			PAN 	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_44_45693_s_312	15337765	2 Because eRF3 interacts with PAN deadenylase, the GDP-bound form of eRF3 might recruit PAN after translation termination to mediate poly	bind
20979	4	6963	6	NULL	NULL	0	NULL	statement 3	NULL		occurs after	NULL				translation	NULL	termination of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_44_45693_s_312	15337765	2 Because eRF3 interacts with PAN deadenylase, the GDP-bound form of eRF3 might recruit PAN after translation termination to mediate poly	bind
25477	1	6964	5	NULL	NULL	0	NULL		NULL		is associated with	NULL	covalently	amino-terminal			NULL	basic	middle rod domains		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_50_35375_s_166	10585405	2 Because the amino-terminal and basic middle rod domains must be covalently associated to stabilize F-actin ( 35) and utrophin lacks the middle rod domain actin binding activity of dystrophin (Figs.  5 and 6), we hypothesize that utrophin may lack the filament-stabilizing activity of dystrophin.	bind
25478	2	6964	5	13	NULL	NULL	NULL	statement 1	Process		stabilizes					F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_50_35375_s_166	10585405	2 Because the amino-terminal and basic middle rod domains must be covalently associated to stabilize F-actin ( 35) and utrophin lacks the middle rod domain actin binding activity of dystrophin (Figs.  5 and 6), we hypothesize that utrophin may lack the filament-stabilizing activity of dystrophin.	bind
25479	3	6964	5	13	NULL	NULL	NULL	utrophin	GP		lacks					dystrophin	GP	actin binding activity of	middle rod domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_50_35375_s_166	10585405	2 Because the amino-terminal and basic middle rod domains must be covalently associated to stabilize F-actin ( 35) and utrophin lacks the middle rod domain actin binding activity of dystrophin (Figs.  5 and 6), we hypothesize that utrophin may lack the filament-stabilizing activity of dystrophin.	bind
25480	4	6964	5	13	NULL	NULL	NULL	utrophin	GP		lack		may			dystrophin	GP	filament-stabilizing activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_50_35375_s_166	10585405	2 Because the amino-terminal and basic middle rod domains must be covalently associated to stabilize F-actin ( 35) and utrophin lacks the middle rod domain actin binding activity of dystrophin (Figs.  5 and 6), we hypothesize that utrophin may lack the filament-stabilizing activity of dystrophin.	bind
25481	5	6964	5	13	NULL	NULL	NULL	statement 3	Process		suggests					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_50_35375_s_166	10585405	2 Because the amino-terminal and basic middle rod domains must be covalently associated to stabilize F-actin ( 35) and utrophin lacks the middle rod domain actin binding activity of dystrophin (Figs.  5 and 6), we hypothesize that utrophin may lack the filament-stabilizing activity of dystrophin.	bind
21187	1	6964	6	NULL	NULL	0	NULL		NULL		associate	NULL	covalently	amino terminal			NULL	basic	middle rod domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_50_35375_s_166	10585405	2 Because the amino-terminal and basic middle rod domains must be covalently associated to stabilize F-actin ( 35) and utrophin lacks the middle rod domain actin binding activity of dystrophin (Figs.  5 and 6), we hypothesize that utrophin may lack the filament-stabilizing activity of dystrophin.	bind
21188	2	6964	6	NULL	NULL	0	NULL	statement 1	NULL		stabilize	NULL				F-actin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_50_35375_s_166	10585405	2 Because the amino-terminal and basic middle rod domains must be covalently associated to stabilize F-actin ( 35) and utrophin lacks the middle rod domain actin binding activity of dystrophin (Figs.  5 and 6), we hypothesize that utrophin may lack the filament-stabilizing activity of dystrophin.	bind
21189	3	6964	6	10	NULL	0	NULL	Utrophin			lack					dystrophin		actin binding activity of 	 middle rod domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_50_35375_s_166	10585405	2 Because the amino-terminal and basic middle rod domains must be covalently associated to stabilize F-actin ( 35) and utrophin lacks the middle rod domain actin binding activity of dystrophin (Figs.  5 and 6), we hypothesize that utrophin may lack the filament-stabilizing activity of dystrophin.	bind
21190	5	6964	6	10	NULL	0	NULL	statement 3			suggest					statement 4					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_50_35375_s_166	10585405	2 Because the amino-terminal and basic middle rod domains must be covalently associated to stabilize F-actin ( 35) and utrophin lacks the middle rod domain actin binding activity of dystrophin (Figs.  5 and 6), we hypothesize that utrophin may lack the filament-stabilizing activity of dystrophin.	bind
21192	4	6964	6	10	NULL	0	NULL	Utrophin			lack		may			dystrophin		filament-stabilizing activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_50_35375_s_166	10585405	2 Because the amino-terminal and basic middle rod domains must be covalently associated to stabilize F-actin ( 35) and utrophin lacks the middle rod domain actin binding activity of dystrophin (Figs.  5 and 6), we hypothesize that utrophin may lack the filament-stabilizing activity of dystrophin.	bind
25482	1	6965	5	13	NULL	NULL	NULL	SRF	GP		plays a role in					cell proliferation	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_16_9755_s_44	9545312	2 Because the role of SRF in cell proliferation and expression of vascular smooth muscle-specific genes is well established, and its DNA-binding element (the CArG box) is rich in adenine and thymine residues, we hypothesized that HMG-I proteins may bind to the CArG box and affect the ability of SRF to bind to DNA and activate transcription.	bind
25483	2	6965	5	13	NULL	NULL	NULL	SRF	GP		plays a role in					vascular smooth muscle-specific genes	Process	expression of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_16_9755_s_44	9545312	2 Because the role of SRF in cell proliferation and expression of vascular smooth muscle-specific genes is well established, and its DNA-binding element (the CArG box) is rich in adenine and thymine residues, we hypothesized that HMG-I proteins may bind to the CArG box and affect the ability of SRF to bind to DNA and activate transcription.	bind
25487	3	6965	5	10	NULL	0	NULL				is rich in				 CArG box				adenine residues		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_16_9755_s_44	9545312	2 Because the role of SRF in cell proliferation and expression of vascular smooth muscle-specific genes is well established, and its DNA-binding element (the CArG box) is rich in adenine and thymine residues, we hypothesized that HMG-I proteins may bind to the CArG box and affect the ability of SRF to bind to DNA and activate transcription.	bind
25488	4	6965	5	10	NULL	0	NULL				is rich in				CArG box				thymine residues		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_16_9755_s_44	9545312	2 Because the role of SRF in cell proliferation and expression of vascular smooth muscle-specific genes is well established, and its DNA-binding element (the CArG box) is rich in adenine and thymine residues, we hypothesized that HMG-I proteins may bind to the CArG box and affect the ability of SRF to bind to DNA and activate transcription.	bind
25489	5	6965	5	13	NULL	NULL	NULL	HMG-I proteins	GP		bind		may							CArG box	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_16_9755_s_44	9545312	2 Because the role of SRF in cell proliferation and expression of vascular smooth muscle-specific genes is well established, and its DNA-binding element (the CArG box) is rich in adenine and thymine residues, we hypothesized that HMG-I proteins may bind to the CArG box and affect the ability of SRF to bind to DNA and activate transcription.	bind
25490	6	6965	5	13	NULL	NULL	NULL	SRF	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_16_9755_s_44	9545312	2 Because the role of SRF in cell proliferation and expression of vascular smooth muscle-specific genes is well established, and its DNA-binding element (the CArG box) is rich in adenine and thymine residues, we hypothesized that HMG-I proteins may bind to the CArG box and affect the ability of SRF to bind to DNA and activate transcription.	bind
25491	7	6965	5	13	NULL	NULL	NULL	statement 6	Process		activates					transcription	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_16_9755_s_44	9545312	2 Because the role of SRF in cell proliferation and expression of vascular smooth muscle-specific genes is well established, and its DNA-binding element (the CArG box) is rich in adenine and thymine residues, we hypothesized that HMG-I proteins may bind to the CArG box and affect the ability of SRF to bind to DNA and activate transcription.	bind
25492	8	6965	5	13	NULL	NULL	NULL	statement 5	Process		affect		may			statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_16_9755_s_44	9545312	2 Because the role of SRF in cell proliferation and expression of vascular smooth muscle-specific genes is well established, and its DNA-binding element (the CArG box) is rich in adenine and thymine residues, we hypothesized that HMG-I proteins may bind to the CArG box and affect the ability of SRF to bind to DNA and activate transcription.	bind
25493	9	6965	5	13	NULL	NULL	NULL	statement 5	Process		affect		may			statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_16_9755_s_44	9545312	2 Because the role of SRF in cell proliferation and expression of vascular smooth muscle-specific genes is well established, and its DNA-binding element (the CArG box) is rich in adenine and thymine residues, we hypothesized that HMG-I proteins may bind to the CArG box and affect the ability of SRF to bind to DNA and activate transcription.	bind
26126	10	6965	5	13	NULL	NULL	NULL	statement 3	Process		occurs simultaneously with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_16_9755_s_44	9545312	2 Because the role of SRF in cell proliferation and expression of vascular smooth muscle-specific genes is well established, and its DNA-binding element (the CArG box) is rich in adenine and thymine residues, we hypothesized that HMG-I proteins may bind to the CArG box and affect the ability of SRF to bind to DNA and activate transcription.	bind
56792	11	6965	5	13	NULL	NULL	NULL	CArG box	NucleicAcid		is a type of					DNA-binding element	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_16_9755_s_44	9545312	2 Because the role of SRF in cell proliferation and expression of vascular smooth muscle-specific genes is well established, and its DNA-binding element (the CArG box) is rich in adenine and thymine residues, we hypothesized that HMG-I proteins may bind to the CArG box and affect the ability of SRF to bind to DNA and activate transcription.	bind
20980	1	6965	6	NULL	NULL	0	NULL	SRF	NULL		plays a role in	NULL				cell proliferation	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_16_9755_s_44	9545312	2 Because the role of SRF in cell proliferation and expression of vascular smooth muscle-specific genes is well established, and its DNA-binding element (the CArG box) is rich in adenine and thymine residues, we hypothesized that HMG-I proteins may bind to the CArG box and affect the ability of SRF to bind to DNA and activate transcription.	bind
20981	2	6965	6	NULL	NULL	0	NULL	SRF	NULL		plays a role in	NULL				vascular smooth muscle-specific genes	NULL	expression of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_16_9755_s_44	9545312	2 Because the role of SRF in cell proliferation and expression of vascular smooth muscle-specific genes is well established, and its DNA-binding element (the CArG box) is rich in adenine and thymine residues, we hypothesized that HMG-I proteins may bind to the CArG box and affect the ability of SRF to bind to DNA and activate transcription.	bind
20982	3	6965	6	NULL	NULL	0	NULL	HMG-I proteins	NULL		bind	NULL	may				NULL			CArG box	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_16_9755_s_44	9545312	2 Because the role of SRF in cell proliferation and expression of vascular smooth muscle-specific genes is well established, and its DNA-binding element (the CArG box) is rich in adenine and thymine residues, we hypothesized that HMG-I proteins may bind to the CArG box and affect the ability of SRF to bind to DNA and activate transcription.	bind
20983	4	6965	6	NULL	NULL	0	NULL		NULL		is rich in	NULL			CArG box	adenine residues	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_16_9755_s_44	9545312	2 Because the role of SRF in cell proliferation and expression of vascular smooth muscle-specific genes is well established, and its DNA-binding element (the CArG box) is rich in adenine and thymine residues, we hypothesized that HMG-I proteins may bind to the CArG box and affect the ability of SRF to bind to DNA and activate transcription.	bind
20984	5	6965	6	NULL	NULL	0	NULL		NULL		is rich in	NULL			CArG box	thymine residues	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_16_9755_s_44	9545312	2 Because the role of SRF in cell proliferation and expression of vascular smooth muscle-specific genes is well established, and its DNA-binding element (the CArG box) is rich in adenine and thymine residues, we hypothesized that HMG-I proteins may bind to the CArG box and affect the ability of SRF to bind to DNA and activate transcription.	bind
20985	6	6965	6	NULL	NULL	0	NULL	SRF	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_16_9755_s_44	9545312	2 Because the role of SRF in cell proliferation and expression of vascular smooth muscle-specific genes is well established, and its DNA-binding element (the CArG box) is rich in adenine and thymine residues, we hypothesized that HMG-I proteins may bind to the CArG box and affect the ability of SRF to bind to DNA and activate transcription.	bind
20986	7	6965	6	NULL	NULL	0	NULL	SRF	NULL		activate	NULL				transcription	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_16_9755_s_44	9545312	2 Because the role of SRF in cell proliferation and expression of vascular smooth muscle-specific genes is well established, and its DNA-binding element (the CArG box) is rich in adenine and thymine residues, we hypothesized that HMG-I proteins may bind to the CArG box and affect the ability of SRF to bind to DNA and activate transcription.	bind
20987	8	6965	6	NULL	NULL	0	NULL	HMG-I proteins	NULL		affect	NULL	may			statement 6	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_16_9755_s_44	9545312	2 Because the role of SRF in cell proliferation and expression of vascular smooth muscle-specific genes is well established, and its DNA-binding element (the CArG box) is rich in adenine and thymine residues, we hypothesized that HMG-I proteins may bind to the CArG box and affect the ability of SRF to bind to DNA and activate transcription.	bind
20988	9	6965	6	NULL	NULL	0	NULL	HMG-I proteins	NULL		affect	NULL	may			statement 7	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_16_9755_s_44	9545312	2 Because the role of SRF in cell proliferation and expression of vascular smooth muscle-specific genes is well established, and its DNA-binding element (the CArG box) is rich in adenine and thymine residues, we hypothesized that HMG-I proteins may bind to the CArG box and affect the ability of SRF to bind to DNA and activate transcription.	bind
25534	10	6965	6	NULL	NULL	0	NULL	statement 4	NULL		occurs simultaneously with	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_16_9755_s_44	9545312	2 Because the role of SRF in cell proliferation and expression of vascular smooth muscle-specific genes is well established, and its DNA-binding element (the CArG box) is rich in adenine and thymine residues, we hypothesized that HMG-I proteins may bind to the CArG box and affect the ability of SRF to bind to DNA and activate transcription.	bind
56793	11	6965	6	10	NULL	0	NULL	CArG box			is a type of					DNA-binding element					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_16_9755_s_44	9545312	2 Because the role of SRF in cell proliferation and expression of vascular smooth muscle-specific genes is well established, and its DNA-binding element (the CArG box) is rich in adenine and thymine residues, we hypothesized that HMG-I proteins may bind to the CArG box and affect the ability of SRF to bind to DNA and activate transcription.	bind
25499	1	6966	5	13	NULL	NULL	NULL	rhotekin protein	GP	human homologue of	associates with		preferentially			RhoC	GP	mutated			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_43_33962_s_123	10940294	2 Besides these artifactual constructs, two different clones corresponded to a cDNA encoding the human homologue of rhotekin, which was originally identified as a protein preferentially associating with a mutated form of RhoC that mimicked the GTP-bound form of this small GTPase ( 25).	bind
31514	2	6966	5	13	NULL	NULL	NULL	RhoC	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_43_33962_s_123	10940294	2 Besides these artifactual constructs, two different clones corresponded to a cDNA encoding the human homologue of rhotekin, which was originally identified as a protein preferentially associating with a mutated form of RhoC that mimicked the GTP-bound form of this small GTPase ( 25).	bind
31515	3	6966	5	13	NULL	NULL	NULL	statement 1	Process		mimics					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_43_33962_s_123	10940294	2 Besides these artifactual constructs, two different clones corresponded to a cDNA encoding the human homologue of rhotekin, which was originally identified as a protein preferentially associating with a mutated form of RhoC that mimicked the GTP-bound form of this small GTPase ( 25).	bind
32234	4	6966	5	13	NULL	NULL	NULL	RhoC	GP		is a type of					small GTPase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_43_33962_s_123	10940294	2 Besides these artifactual constructs, two different clones corresponded to a cDNA encoding the human homologue of rhotekin, which was originally identified as a protein preferentially associating with a mutated form of RhoC that mimicked the GTP-bound form of this small GTPase ( 25).	bind
21193	1	6966	6	10	NULL	0	NULL	rhotekin		human homologue of	associate		preferentially			RhoC		mutant			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_43_33962_s_123	10940294	2 Besides these artifactual constructs, two different clones corresponded to a cDNA encoding the human homologue of rhotekin, which was originally identified as a protein preferentially associating with a mutated form of RhoC that mimicked the GTP-bound form of this small GTPase ( 25).	bind
21194	2	6966	6	10	NULL	0	NULL	RhoC			is a type of					small GTPase					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_43_33962_s_123	10940294	2 Besides these artifactual constructs, two different clones corresponded to a cDNA encoding the human homologue of rhotekin, which was originally identified as a protein preferentially associating with a mutated form of RhoC that mimicked the GTP-bound form of this small GTPase ( 25).	bind
21195	3	6966	6	NULL	NULL	0	NULL	RhoC	NULL		bind	NULL				GTP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_43_33962_s_123	10940294	2 Besides these artifactual constructs, two different clones corresponded to a cDNA encoding the human homologue of rhotekin, which was originally identified as a protein preferentially associating with a mutated form of RhoC that mimicked the GTP-bound form of this small GTPase ( 25).	bind
21196	4	6966	6	NULL	NULL	0	NULL	statement 1	NULL		mimicks	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_43_33962_s_123	10940294	2 Besides these artifactual constructs, two different clones corresponded to a cDNA encoding the human homologue of rhotekin, which was originally identified as a protein preferentially associating with a mutated form of RhoC that mimicked the GTP-bound form of this small GTPase ( 25).	bind
25500	1	6967	5	13	NULL	NULL	NULL	Bet1p	GP		bind		directly			Sec24p	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_26_27225_s_250	15123693	2 Bet1p also binds directly to Sec24p, and its COPII binding motif is occluded when assembled into SNARE complexes, suggesting that Bet1p is also packaged into COPII vesicles in a free form ( ).	bind
25501	2	6967	5	13	NULL	NULL	NULL	Bet1p	GP		is occluded when			COPII binding motif		SNARE complexes	GP	assembled into			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_26_27225_s_250	15123693	2 Bet1p also binds directly to Sec24p, and its COPII binding motif is occluded when assembled into SNARE complexes, suggesting that Bet1p is also packaged into COPII vesicles in a free form ( ).	bind
25502	3	6967	5	13	NULL	NULL	NULL	Bet1p	GP	free form	is packaged into					COPII vesicles	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_26_27225_s_250	15123693	2 Bet1p also binds directly to Sec24p, and its COPII binding motif is occluded when assembled into SNARE complexes, suggesting that Bet1p is also packaged into COPII vesicles in a free form ( ).	bind
25503	4	6967	5	13	NULL	NULL	NULL	statement 2	Process		suggests					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_26_27225_s_250	15123693	2 Bet1p also binds directly to Sec24p, and its COPII binding motif is occluded when assembled into SNARE complexes, suggesting that Bet1p is also packaged into COPII vesicles in a free form ( ).	bind
20989	1	6967	6	NULL	NULL	0	NULL	Bet1p	NULL		bind	NULL	directly			Sec24p	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_26_27225_s_250	15123693	2 Bet1p also binds directly to Sec24p, and its COPII binding motif is occluded when assembled into SNARE complexes, suggesting that Bet1p is also packaged into COPII vesicles in a free form ( ).	bind
20990	2	6967	6	NULL	NULL	0	NULL	Bet1p	NULL		is occluded when	NULL		COPII binding motif		SNARE complexs	NULL	assembled into			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_26_27225_s_250	15123693	2 Bet1p also binds directly to Sec24p, and its COPII binding motif is occluded when assembled into SNARE complexes, suggesting that Bet1p is also packaged into COPII vesicles in a free form ( ).	bind
20991	3	6967	6	NULL	NULL	0	NULL	Bet1p	NULL	free form	packaged into	NULL				COPII vesicles	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_26_27225_s_250	15123693	2 Bet1p also binds directly to Sec24p, and its COPII binding motif is occluded when assembled into SNARE complexes, suggesting that Bet1p is also packaged into COPII vesicles in a free form ( ).	bind
30690	4	6967	6	NULL	NULL	0	NULL	statement 2	NULL		suggests	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_26_27225_s_250	15123693	2 Bet1p also binds directly to Sec24p, and its COPII binding motif is occluded when assembled into SNARE complexes, suggesting that Bet1p is also packaged into COPII vesicles in a free form ( ).	bind
25504	1	6968	5	13	NULL	NULL	NULL	Bla g 2	GP		is not expressed in					P. americana	Organism				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_33_20907_s_142	9252418	2 Bla g 2 and Bla g 4 are not expressed in  P. americana and recent results showed that  P. americana extracts did not inhibit IgE Ab binding to Bla g 5 in RIA ( 12,  13).	bind
25505	2	6968	5	13	NULL	NULL	NULL	Bla g 4	GP		is not expressed in					P. americana	Organism				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_33_20907_s_142	9252418	2 Bla g 2 and Bla g 4 are not expressed in  P. americana and recent results showed that  P. americana extracts did not inhibit IgE Ab binding to Bla g 5 in RIA ( 12,  13).	bind
25506	3	6968	5	13	NULL	NULL	NULL	IgE Ab	GP		bind					Bla g 5	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_33_20907_s_142	9252418	2 Bla g 2 and Bla g 4 are not expressed in  P. americana and recent results showed that  P. americana extracts did not inhibit IgE Ab binding to Bla g 5 in RIA ( 12,  13).	bind
25507	4	6968	5	13	NULL	NULL	NULL	P. americana extracts	Cell		does not inhibit					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_33_20907_s_142	9252418	2 Bla g 2 and Bla g 4 are not expressed in  P. americana and recent results showed that  P. americana extracts did not inhibit IgE Ab binding to Bla g 5 in RIA ( 12,  13).	bind
20992	1	6968	6	NULL	NULL	0	NULL	Bla g2	NULL		is not expressed in	NULL				P. americana	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_33_20907_s_142	9252418	2 Bla g 2 and Bla g 4 are not expressed in  P. americana and recent results showed that  P. americana extracts did not inhibit IgE Ab binding to Bla g 5 in RIA ( 12,  13).	bind
20993	2	6968	6	NULL	NULL	0	NULL	Bla g4	NULL		is not expressed in	NULL				P. americana	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_33_20907_s_142	9252418	2 Bla g 2 and Bla g 4 are not expressed in  P. americana and recent results showed that  P. americana extracts did not inhibit IgE Ab binding to Bla g 5 in RIA ( 12,  13).	bind
20994	3	6968	6	NULL	NULL	0	NULL	IgE Ab	NULL		bind	NULL				Bla g5	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_33_20907_s_142	9252418	2 Bla g 2 and Bla g 4 are not expressed in  P. americana and recent results showed that  P. americana extracts did not inhibit IgE Ab binding to Bla g 5 in RIA ( 12,  13).	bind
20995	4	6968	6	NULL	NULL	0	NULL	P. americana extracts	NULL		did not inhibit	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_33_20907_s_142	9252418	2 Bla g 2 and Bla g 4 are not expressed in  P. americana and recent results showed that  P. americana extracts did not inhibit IgE Ab binding to Bla g 5 in RIA ( 12,  13).	bind
25508	1	6970	5	13	NULL	NULL	NULL	nuclear receptor superfamily members	GP		is a class of					transcription factors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_1_663_s_20	8995310	2 Both steroid hormones and RA are triggers of ligand-dependent activation of their respective receptors, which are members of the nuclear receptor superfamily, a class of transcription factors that specifically bind to  cis-elements in the regulatory regions of given genes ( 15).	bind
25509	2	6970	5	13	NULL	NULL	NULL	nuclear receptor superfamily members	GP		bind					genes	GP			 cis-elements in the regulatory regions	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_1_663_s_20	8995310	2 Both steroid hormones and RA are triggers of ligand-dependent activation of their respective receptors, which are members of the nuclear receptor superfamily, a class of transcription factors that specifically bind to  cis-elements in the regulatory regions of given genes ( 15).	bind
31516	3	6970	5	13	NULL	NULL	NULL	steroid hormones	Chemical		triggers					nuclear receptor superfamily members	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_1_663_s_20	8995310	2 Both steroid hormones and RA are triggers of ligand-dependent activation of their respective receptors, which are members of the nuclear receptor superfamily, a class of transcription factors that specifically bind to  cis-elements in the regulatory regions of given genes ( 15).	bind
31517	4	6970	5	13	NULL	NULL	NULL	statement 3	Process		is dependent on					ligand	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_1_663_s_20	8995310	2 Both steroid hormones and RA are triggers of ligand-dependent activation of their respective receptors, which are members of the nuclear receptor superfamily, a class of transcription factors that specifically bind to  cis-elements in the regulatory regions of given genes ( 15).	bind
56794	5	6970	5	13	NULL	NULL	NULL	RA	Chemical		triggers					nuclear receptor superfamily member	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_1_663_s_20	8995310	2 Both steroid hormones and RA are triggers of ligand-dependent activation of their respective receptors, which are members of the nuclear receptor superfamily, a class of transcription factors that specifically bind to  cis-elements in the regulatory regions of given genes ( 15).	bind
56795	6	6970	5	13	NULL	NULL	NULL	statement 5	Process		is dependent on					ligand	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_1_663_s_20	8995310	2 Both steroid hormones and RA are triggers of ligand-dependent activation of their respective receptors, which are members of the nuclear receptor superfamily, a class of transcription factors that specifically bind to  cis-elements in the regulatory regions of given genes ( 15).	bind
21197	1	6970	6	10	NULL	0	NULL	nuclear receptor superfamily		members of	is a class of					transcription factors					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_1_663_s_20	8995310	2 Both steroid hormones and RA are triggers of ligand-dependent activation of their respective receptors, which are members of the nuclear receptor superfamily, a class of transcription factors that specifically bind to  cis-elements in the regulatory regions of given genes ( 15).	bind
21198	2	6970	6	NULL	NULL	0	NULL	transcription factors	NULL		bind	NULL	specifically			gene	NULL			cis-elements in the regulatory region	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_1_663_s_20	8995310	2 Both steroid hormones and RA are triggers of ligand-dependent activation of their respective receptors, which are members of the nuclear receptor superfamily, a class of transcription factors that specifically bind to  cis-elements in the regulatory regions of given genes ( 15).	bind
21199	3	6970	6	NULL	NULL	0	NULL	steroid hormone	NULL		triggers	NULL				members of nuclear receptor superfamily	NULL	activation of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_1_663_s_20	8995310	2 Both steroid hormones and RA are triggers of ligand-dependent activation of their respective receptors, which are members of the nuclear receptor superfamily, a class of transcription factors that specifically bind to  cis-elements in the regulatory regions of given genes ( 15).	bind
21200	4	6970	6	NULL	NULL	0	NULL	RA	NULL		triggers	NULL				members of nuclear receptor superfamily	NULL	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_1_663_s_20	8995310	2 Both steroid hormones and RA are triggers of ligand-dependent activation of their respective receptors, which are members of the nuclear receptor superfamily, a class of transcription factors that specifically bind to  cis-elements in the regulatory regions of given genes ( 15).	bind
21201	5	6970	6	NULL	NULL	0	NULL	statement 3	NULL		is dependent on	NULL				ligand	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_1_663_s_20	8995310	2 Both steroid hormones and RA are triggers of ligand-dependent activation of their respective receptors, which are members of the nuclear receptor superfamily, a class of transcription factors that specifically bind to  cis-elements in the regulatory regions of given genes ( 15).	bind
21212	6	6970	6	NULL	NULL	0	NULL	statement 4	NULL		is dependent on	NULL				ligand	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_1_663_s_20	8995310	2 Both steroid hormones and RA are triggers of ligand-dependent activation of their respective receptors, which are members of the nuclear receptor superfamily, a class of transcription factors that specifically bind to  cis-elements in the regulatory regions of given genes ( 15).	bind
25516	1	6971	5	13	NULL	NULL	NULL	CC-G24	GP		bind		specifically			bFcgamma2R	GP				NULL	in bovine neutrophils	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_51_47794_s_69	11641395	2 CC-G24 bound specifically to bFcgamma2R expressed at high levels on bovine neutrophils (Fig.  1,  panel A).	bind
31518	2	6971	5	13	NULL	NULL	NULL	bFcgamma2R	GP	high levels of	expressed on					neutrophils	Cell	bovine			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_51_47794_s_69	11641395	2 CC-G24 bound specifically to bFcgamma2R expressed at high levels on bovine neutrophils (Fig.  1,  panel A).	bind
20996	1	6971	6	10	NULL	0	NULL	bFcgamma2R		high levels of	expressed on					neutrophils		bovine			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_51_47794_s_69	11641395	2 CC-G24 bound specifically to bFcgamma2R expressed at high levels on bovine neutrophils (Fig.  1,  panel A).	bind
20997	2	6971	6	10	NULL	0	NULL	CC-G24			bind		specifically			bFcgamma2R					NULL	bovine neutrophils	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_51_47794_s_69	11641395	2 CC-G24 bound specifically to bFcgamma2R expressed at high levels on bovine neutrophils (Fig.  1,  panel A).	bind
28988	1	6972	5	13	NULL	NULL	NULL	RPs mRNAs	NucleicAcid	change of levels of	does not change		significantly			Rap1p	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_19_13235_s_253	10224082	2 Conditions that produce changes in the levels of mRNAs encoding RPs do not significantly change the levels of expression of Rap1p ( 16), or change the binding affinities of Rap1p and Abf1p ( 12,  14,  16).	bind
28989	2	6972	5	13	NULL	NULL	NULL	RPs mRNAs	NucleicAcid	change of levels of	does not change					Rap1p	GP	binding affinities of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_19_13235_s_253	10224082	2 Conditions that produce changes in the levels of mRNAs encoding RPs do not significantly change the levels of expression of Rap1p ( 16), or change the binding affinities of Rap1p and Abf1p ( 12,  14,  16).	bind
28990	3	6972	5	13	NULL	NULL	NULL	RPs mRNAs	NucleicAcid	change of levels of	does not change					Abf1p	GP	binding affinities of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_19_13235_s_253	10224082	2 Conditions that produce changes in the levels of mRNAs encoding RPs do not significantly change the levels of expression of Rap1p ( 16), or change the binding affinities of Rap1p and Abf1p ( 12,  14,  16).	bind
20998	1	6972	6	13	NULL	NULL	NULL	RPs mRNAs	NucleicAcid	change of levels of 	does not change		significantly			Rap1p	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_19_13235_s_253	10224082	2 Conditions that produce changes in the levels of mRNAs encoding RPs do not significantly change the levels of expression of Rap1p ( 16), or change the binding affinities of Rap1p and Abf1p ( 12,  14,  16).	bind
30691	2	6972	6	10	NULL	0	NULL	RPs mRNAs	NULL	change of levels of	does not change	NULL				Rap1p	NULL	binding affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_19_13235_s_253	10224082	2 Conditions that produce changes in the levels of mRNAs encoding RPs do not significantly change the levels of expression of Rap1p ( 16), or change the binding affinities of Rap1p and Abf1p ( 12,  14,  16).	bind
30692	3	6972	6	10	NULL	0	NULL	RPs mRNAs	NULL	change of levels of	does not change	NULL				Abf1p	NULL	binding affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_19_13235_s_253	10224082	2 Conditions that produce changes in the levels of mRNAs encoding RPs do not significantly change the levels of expression of Rap1p ( 16), or change the binding affinities of Rap1p and Abf1p ( 12,  14,  16).	bind
25517	1	6973	5	13	NULL	NULL	NULL	paxillin	GP		associates with					PTP-PEST	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_30_22736_s_226	10781578	2 Consequently, our data suggest that alpha4 can bind simultaneously to paxillin that is associated with PTP-PEST or FAK.	bind
25518	2	6973	5	13	NULL	NULL	NULL	paxillin	GP		associate with					FAK	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_30_22736_s_226	10781578	2 Consequently, our data suggest that alpha4 can bind simultaneously to paxillin that is associated with PTP-PEST or FAK.	bind
25519	3	6973	5	13	NULL	NULL	NULL	alpha4	GP		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_30_22736_s_226	10781578	2 Consequently, our data suggest that alpha4 can bind simultaneously to paxillin that is associated with PTP-PEST or FAK.	bind
25520	4	6973	5	13	NULL	NULL	NULL	alpha4	GP		bind					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_30_22736_s_226	10781578	2 Consequently, our data suggest that alpha4 can bind simultaneously to paxillin that is associated with PTP-PEST or FAK.	bind
25521	5	6973	5	13	NULL	NULL	NULL	statement 3	Process		occurs simultaneously with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_30_22736_s_226	10781578	2 Consequently, our data suggest that alpha4 can bind simultaneously to paxillin that is associated with PTP-PEST or FAK.	bind
56796	6	6973	5	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_30_22736_s_226	10781578	2 Consequently, our data suggest that alpha4 can bind simultaneously to paxillin that is associated with PTP-PEST or FAK.	bind
20999	1	6973	6	NULL	NULL	0	NULL	paxillin	NULL		is associated with	NULL				PTP-PEST	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_30_22736_s_226	10781578	2 Consequently, our data suggest that alpha4 can bind simultaneously to paxillin that is associated with PTP-PEST or FAK.	bind
21000	2	6973	6	NULL	NULL	0	NULL	Paxillin	NULL		is associated with	NULL				FAK	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_30_22736_s_226	10781578	2 Consequently, our data suggest that alpha4 can bind simultaneously to paxillin that is associated with PTP-PEST or FAK.	bind
21001	3	6973	6	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_30_22736_s_226	10781578	2 Consequently, our data suggest that alpha4 can bind simultaneously to paxillin that is associated with PTP-PEST or FAK.	bind
21002	4	6973	6	NULL	NULL	0	NULL	alpha4	NULL		bind	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_30_22736_s_226	10781578	2 Consequently, our data suggest that alpha4 can bind simultaneously to paxillin that is associated with PTP-PEST or FAK.	bind
21003	5	6973	6	NULL	NULL	0	NULL	alpha4	NULL		bind	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_30_22736_s_226	10781578	2 Consequently, our data suggest that alpha4 can bind simultaneously to paxillin that is associated with PTP-PEST or FAK.	bind
30695	6	6973	6	NULL	NULL	0	NULL	statement 4	NULL		occurs simultaneously with	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_30_22736_s_226	10781578	2 Consequently, our data suggest that alpha4 can bind simultaneously to paxillin that is associated with PTP-PEST or FAK.	bind
25522	1	6974	5	13	NULL	NULL	NULL	CrkL	GP		bind		constitutively			C3G guanine nucleotide exchange factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_46_30630_s_294	9804835	2 CrkL constitutively binds the C3G guanine nucleotide exchange factor ( 15,  34), which has been implicated in activation of the Rap1 GTPase ( 35) and the c-Jun N-terminal kinase ( 36).	bind
25523	2	6974	5	13	NULL	NULL	NULL	C3G guanine nucleotide exchange factor	GP		is implicated in					Rap1 GTPase	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_46_30630_s_294	9804835	2 CrkL constitutively binds the C3G guanine nucleotide exchange factor ( 15,  34), which has been implicated in activation of the Rap1 GTPase ( 35) and the c-Jun N-terminal kinase ( 36).	bind
25525	3	6974	5	13	NULL	NULL	NULL	C3G guanine nucleotide exchange factor	GP		is implicated in					c-Jun N-terminal kinase	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_46_30630_s_294	9804835	2 CrkL constitutively binds the C3G guanine nucleotide exchange factor ( 15,  34), which has been implicated in activation of the Rap1 GTPase ( 35) and the c-Jun N-terminal kinase ( 36).	bind
21004	1	6974	6	NULL	NULL	0	NULL	CrkL	NULL		bind	NULL	constitutively			C3G guanine nucleotide exchange factor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_46_30630_s_294	9804835	2 CrkL constitutively binds the C3G guanine nucleotide exchange factor ( 15,  34), which has been implicated in activation of the Rap1 GTPase ( 35) and the c-Jun N-terminal kinase ( 36).	bind
21005	2	6974	6	NULL	NULL	0	NULL	C3G guanine nucleotide exchange factor	NULL		is involved in	NULL				Rap1 GTPase	NULL	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_46_30630_s_294	9804835	2 CrkL constitutively binds the C3G guanine nucleotide exchange factor ( 15,  34), which has been implicated in activation of the Rap1 GTPase ( 35) and the c-Jun N-terminal kinase ( 36).	bind
21006	3	6974	6	NULL	NULL	0	NULL	C3G guanine nucleotide exchange factor	NULL		is involved in	NULL				c-Jun N-terminal kinase	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_46_30630_s_294	9804835	2 CrkL constitutively binds the C3G guanine nucleotide exchange factor ( 15,  34), which has been implicated in activation of the Rap1 GTPase ( 35) and the c-Jun N-terminal kinase ( 36).	bind
25527	1	6975	5	13	NULL	NULL	NULL			deletion of	results in				CREB/cAMP-response element modulator protein binding site	enhancer activity	NucleicAcid	complete loss of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_35_32489_s_252	11432851	2 Deletion or mutation of the CREB/cAMP-response element modulator protein binding site results in complete loss of enhancer activity.	bind
25528	2	6975	5	13	NULL	NULL	NULL			mutation of	results in				CREB/cAMP-response element modulator protein binding site	enhancer activity	NucleicAcid	complete loss of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_35_32489_s_252	11432851	2 Deletion or mutation of the CREB/cAMP-response element modulator protein binding site results in complete loss of enhancer activity.	bind
25529	3	6975	5	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_35_32489_s_252	11432851	2 Deletion or mutation of the CREB/cAMP-response element modulator protein binding site results in complete loss of enhancer activity.	bind
21229	1	6975	6	NULL	NULL	0	NULL		NULL	deletion of	results in	NULL			CREB/cAMP-response element modulator protein binding site	enhancer activity	NULL	complete loss of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_35_32489_s_252	11432851	2 Deletion or mutation of the CREB/cAMP-response element modulator protein binding site results in complete loss of enhancer activity.	bind
30711	2	6975	6	NULL	NULL	0	NULL		NULL	mutation of	results in	NULL			CREB/cAMP-response element modulator protein binding site	enhancer activity	NULL	complete loss of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_35_32489_s_252	11432851	2 Deletion or mutation of the CREB/cAMP-response element modulator protein binding site results in complete loss of enhancer activity.	bind
56797	3	6975	6	10	NULL	0	NULL	statement 1			is an alternative to					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_35_32489_s_252	11432851	2 Deletion or mutation of the CREB/cAMP-response element modulator protein binding site results in complete loss of enhancer activity.	bind
25530	1	6976	5	13	NULL	NULL	NULL	Cya-RalF	GP		is delivered into					host cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_2_1392_s_84	15520000	2 Delivery of a Cya-RalF fusion protein into host cells results in calmodulin binding to the adenylate cyclase enzyme, resulting in the production of cAMP.	bind
25531	2	6976	5	13	NULL	NULL	NULL	calmodulin	GP		bind					adenylate cyclase enzyme	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_2_1392_s_84	15520000	2 Delivery of a Cya-RalF fusion protein into host cells results in calmodulin binding to the adenylate cyclase enzyme, resulting in the production of cAMP.	bind
25532	3	6976	5	13	NULL	NULL	NULL	statement 1	Process		results in					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_2_1392_s_84	15520000	2 Delivery of a Cya-RalF fusion protein into host cells results in calmodulin binding to the adenylate cyclase enzyme, resulting in the production of cAMP.	bind
25533	4	6976	5	13	NULL	NULL	NULL	statement 3	Process		results in					cAMP	Chemical	production of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_2_1392_s_84	15520000	2 Delivery of a Cya-RalF fusion protein into host cells results in calmodulin binding to the adenylate cyclase enzyme, resulting in the production of cAMP.	bind
44812	5	6976	5	13	NULL	NULL	NULL	Cya-RalF	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_2_1392_s_84	15520000	2 Delivery of a Cya-RalF fusion protein into host cells results in calmodulin binding to the adenylate cyclase enzyme, resulting in the production of cAMP.	bind
21027	1	6976	6	NULL	NULL	0	NULL	Calmodulin	NULL		bind	NULL				adenylate cyclase enzyme	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_2_1392_s_84	15520000	2 Delivery of a Cya-RalF fusion protein into host cells results in calmodulin binding to the adenylate cyclase enzyme, resulting in the production of cAMP.	bind
21028	2	6976	6	10	NULL	0	NULL	Cya-RalF	NULL	delivery of	into	NULL				host cells	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_2_1392_s_84	15520000	2 Delivery of a Cya-RalF fusion protein into host cells results in calmodulin binding to the adenylate cyclase enzyme, resulting in the production of cAMP.	bind
21029	3	6976	6	NULL	NULL	0	NULL	statement 2	NULL		results in	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_2_1392_s_84	15520000	2 Delivery of a Cya-RalF fusion protein into host cells results in calmodulin binding to the adenylate cyclase enzyme, resulting in the production of cAMP.	bind
21030	4	6976	6	NULL	NULL	0	NULL	statement 1	NULL		results in	NULL				cAMP	NULL	production of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_2_1392_s_84	15520000	2 Delivery of a Cya-RalF fusion protein into host cells results in calmodulin binding to the adenylate cyclase enzyme, resulting in the production of cAMP.	bind
44816	5	6976	6	10	NULL	0	NULL	Cya-RalF	NULL		is a type of	NULL				fusion protein	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_2_1392_s_84	15520000	2 Delivery of a Cya-RalF fusion protein into host cells results in calmodulin binding to the adenylate cyclase enzyme, resulting in the production of cAMP.	bind
25752	1	6977	5	13	NULL	NULL	NULL	ATP	Chemical		bind					Arp2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_50_46689_s_135	11598103	2 Detailed balance, however, implies that if the affinity of ATP for Arp2 is enhanced by WA, a structural change of the WA.Arp2 complex, linked to enhanced interaction of WA with Arp2, must accompany ATP binding to Arp2.	bind
25753	2	6977	5	13	NULL	NULL	NULL	WA	GP		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_50_46689_s_135	11598103	2 Detailed balance, however, implies that if the affinity of ATP for Arp2 is enhanced by WA, a structural change of the WA.Arp2 complex, linked to enhanced interaction of WA with Arp2, must accompany ATP binding to Arp2.	bind
25754	3	6977	5	13	NULL	NULL	NULL	statement 2	Process		leads to					WA.Arp2 complex	GP	structural change of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_50_46689_s_135	11598103	2 Detailed balance, however, implies that if the affinity of ATP for Arp2 is enhanced by WA, a structural change of the WA.Arp2 complex, linked to enhanced interaction of WA with Arp2, must accompany ATP binding to Arp2.	bind
25755	4	6977	5	13	NULL	NULL	NULL	WA	GP		interacts with					Arp2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_50_46689_s_135	11598103	2 Detailed balance, however, implies that if the affinity of ATP for Arp2 is enhanced by WA, a structural change of the WA.Arp2 complex, linked to enhanced interaction of WA with Arp2, must accompany ATP binding to Arp2.	bind
25756	5	6977	5	13	NULL	NULL	NULL	statement 3	Process		is linked to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_50_46689_s_135	11598103	2 Detailed balance, however, implies that if the affinity of ATP for Arp2 is enhanced by WA, a structural change of the WA.Arp2 complex, linked to enhanced interaction of WA with Arp2, must accompany ATP binding to Arp2.	bind
25758	6	6977	5	13	NULL	NULL	NULL	statement 1	Process		accompanies					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_50_46689_s_135	11598103	2 Detailed balance, however, implies that if the affinity of ATP for Arp2 is enhanced by WA, a structural change of the WA.Arp2 complex, linked to enhanced interaction of WA with Arp2, must accompany ATP binding to Arp2.	bind
21031	1	6977	6	10	NULL	0	NULL	ATP			bind					Arp2					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_50_46689_s_135	11598103	2 Detailed balance, however, implies that if the affinity of ATP for Arp2 is enhanced by WA, a structural change of the WA.Arp2 complex, linked to enhanced interaction of WA with Arp2, must accompany ATP binding to Arp2.	bind
21222	2	6977	6	NULL	NULL	0	NULL	WA	NULL		enhances	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_50_46689_s_135	11598103	2 Detailed balance, however, implies that if the affinity of ATP for Arp2 is enhanced by WA, a structural change of the WA.Arp2 complex, linked to enhanced interaction of WA with Arp2, must accompany ATP binding to Arp2.	bind
21224	3	6977	6	NULL	NULL	0	NULL	WA	NULL		interacts with	NULL				Arp2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_50_46689_s_135	11598103	2 Detailed balance, however, implies that if the affinity of ATP for Arp2 is enhanced by WA, a structural change of the WA.Arp2 complex, linked to enhanced interaction of WA with Arp2, must accompany ATP binding to Arp2.	bind
21228	4	6977	6	10	NULL	0	NULL	statement 1			accompanies					statement 3					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_50_46689_s_135	11598103	2 Detailed balance, however, implies that if the affinity of ATP for Arp2 is enhanced by WA, a structural change of the WA.Arp2 complex, linked to enhanced interaction of WA with Arp2, must accompany ATP binding to Arp2.	bind
56898	5	6977	6	10	NULL	0	NULL	statement 2			leads to					WA.Arp2 complex		structural change of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_50_46689_s_135	11598103	2 Detailed balance, however, implies that if the affinity of ATP for Arp2 is enhanced by WA, a structural change of the WA.Arp2 complex, linked to enhanced interaction of WA with Arp2, must accompany ATP binding to Arp2.	bind
56899	6	6977	6	10	NULL	0	NULL	statement 5			is linked to					statement 3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_50_46689_s_135	11598103	2 Detailed balance, however, implies that if the affinity of ATP for Arp2 is enhanced by WA, a structural change of the WA.Arp2 complex, linked to enhanced interaction of WA with Arp2, must accompany ATP binding to Arp2.	bind
25760	1	6979	5	13	NULL	NULL	NULL	d[Cha(4)]AVP	Chemical		bind					hV(1b) receptors	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_br-j-pharmacol_146_5_16158071_s_5	16158071	2 d[Cha(4)]AVP bound to hV(1b) receptors and hOT receptors  with pK(i) values of 9.68+/-0.06 and 7.68+/-0.09, respectively.	bind
25761	2	6979	5	13	NULL	NULL	NULL	d[Cha(4)]AVP	Chemical		bind					hOT receptors	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_br-j-pharmacol_146_5_16158071_s_5	16158071	2 d[Cha(4)]AVP bound to hV(1b) receptors and hOT receptors  with pK(i) values of 9.68+/-0.06 and 7.68+/-0.09, respectively.	bind
21032	1	6979	6	10	NULL	0	NULL	d[Cha(4)]AVP			bind					hV(1b) receptors					NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_br-j-pharmacol_146_5_16158071_s_5	16158071	2 d[Cha(4)]AVP bound to hV(1b) receptors and hOT receptors  with pK(i) values of 9.68+/-0.06 and 7.68+/-0.09, respectively.	bind
21033	2	6979	6	10	NULL	0	NULL	d[Cha(4)]AVP			bind					hOT receptors					NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_br-j-pharmacol_146_5_16158071_s_5	16158071	2 d[Cha(4)]AVP bound to hV(1b) receptors and hOT receptors  with pK(i) values of 9.68+/-0.06 and 7.68+/-0.09, respectively.	bind
25762	1	6980	5	13	NULL	NULL	NULL	E3BP	GP		contains								inner domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_10_6361_s_29	9045657	2 E3BP is also composed of three linker-connected domains (an inner domain that binds to the I domain of E2, an E3-binding domain, and a lipoyl domain) ( 3,  4,  13,  27).	bind
25763	2	6980	5	13	NULL	NULL	NULL	E3BP	GP		bind			inner domain		E2	GP		I domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_10_6361_s_29	9045657	2 E3BP is also composed of three linker-connected domains (an inner domain that binds to the I domain of E2, an E3-binding domain, and a lipoyl domain) ( 3,  4,  13,  27).	bind
31519	3	6980	5	13	NULL	NULL	NULL	E3BP	GP		contains								E3-binding domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_10_6361_s_29	9045657	2 E3BP is also composed of three linker-connected domains (an inner domain that binds to the I domain of E2, an E3-binding domain, and a lipoyl domain) ( 3,  4,  13,  27).	bind
31520	4	6980	5	13	NULL	NULL	NULL	E3BP	GP		contains								lipoyl domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_10_6361_s_29	9045657	2 E3BP is also composed of three linker-connected domains (an inner domain that binds to the I domain of E2, an E3-binding domain, and a lipoyl domain) ( 3,  4,  13,  27).	bind
21034	1	6980	6	NULL	NULL	0	NULL	E3BP	NULL		contains	NULL					NULL		inner domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_10_6361_s_29	9045657	2 E3BP is also composed of three linker-connected domains (an inner domain that binds to the I domain of E2, an E3-binding domain, and a lipoyl domain) ( 3,  4,  13,  27).	bind
21035	2	6980	6	NULL	NULL	0	NULL	E3BP	NULL		contains	NULL					NULL		E3-binding domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_10_6361_s_29	9045657	2 E3BP is also composed of three linker-connected domains (an inner domain that binds to the I domain of E2, an E3-binding domain, and a lipoyl domain) ( 3,  4,  13,  27).	bind
21036	3	6980	6	NULL	NULL	0	NULL	E3BP	NULL		contains	NULL					NULL		lipoyl domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_10_6361_s_29	9045657	2 E3BP is also composed of three linker-connected domains (an inner domain that binds to the I domain of E2, an E3-binding domain, and a lipoyl domain) ( 3,  4,  13,  27).	bind
21037	4	6980	6	NULL	NULL	0	NULL	E3BP	NULL		bind	NULL		inner domain		E2	NULL		I domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_10_6361_s_29	9045657	2 E3BP is also composed of three linker-connected domains (an inner domain that binds to the I domain of E2, an E3-binding domain, and a lipoyl domain) ( 3,  4,  13,  27).	bind
25799	1	6981	5	13	NULL	NULL	NULL	Golgi p180	GP		bind					Cdc42	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_35_22537_s_105	9712880	2 Finally, similar to the cytosolic IQGAPs ( 21), binding of Golgi p180 to Cdc42 was competed by the p21-activated kinase, a putative target for Cdc42, but not by the Cdc42-GAP (data not shown).	bind
25800	2	6981	5	13	NULL	NULL	NULL	p21-activated kinase	GP		bind					Cdc42	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_35_22537_s_105	9712880	2 Finally, similar to the cytosolic IQGAPs ( 21), binding of Golgi p180 to Cdc42 was competed by the p21-activated kinase, a putative target for Cdc42, but not by the Cdc42-GAP (data not shown).	bind
25801	3	6981	5	13	NULL	NULL	NULL	statement 2	Process		competes with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_35_22537_s_105	9712880	2 Finally, similar to the cytosolic IQGAPs ( 21), binding of Golgi p180 to Cdc42 was competed by the p21-activated kinase, a putative target for Cdc42, but not by the Cdc42-GAP (data not shown).	bind
25802	4	6981	5	13	NULL	NULL	NULL	p21-activated kinase	GP		is target for		putative			Cdc42	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_35_22537_s_105	9712880	2 Finally, similar to the cytosolic IQGAPs ( 21), binding of Golgi p180 to Cdc42 was competed by the p21-activated kinase, a putative target for Cdc42, but not by the Cdc42-GAP (data not shown).	bind
25803	5	6981	5	13	NULL	NULL	NULL	p21-activated kinase	GP		is not target for					Cdc42-GAP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_35_22537_s_105	9712880	2 Finally, similar to the cytosolic IQGAPs ( 21), binding of Golgi p180 to Cdc42 was competed by the p21-activated kinase, a putative target for Cdc42, but not by the Cdc42-GAP (data not shown).	bind
21038	1	6981	6	NULL	NULL	0	NULL	golgi p180	NULL		bind	NULL				Cdc42	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_35_22537_s_105	9712880	2 Finally, similar to the cytosolic IQGAPs ( 21), binding of Golgi p180 to Cdc42 was competed by the p21-activated kinase, a putative target for Cdc42, but not by the Cdc42-GAP (data not shown).	bind
21039	2	6981	6	NULL	NULL	0	NULL	p21-activated kinase	NULL		bind	NULL				Cdc42	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_35_22537_s_105	9712880	2 Finally, similar to the cytosolic IQGAPs ( 21), binding of Golgi p180 to Cdc42 was competed by the p21-activated kinase, a putative target for Cdc42, but not by the Cdc42-GAP (data not shown).	bind
21040	3	6981	6	NULL	NULL	0	NULL	statement 1	NULL		competes	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_35_22537_s_105	9712880	2 Finally, similar to the cytosolic IQGAPs ( 21), binding of Golgi p180 to Cdc42 was competed by the p21-activated kinase, a putative target for Cdc42, but not by the Cdc42-GAP (data not shown).	bind
30714	4	6981	6	NULL	NULL	0	NULL	p21-activated kinase	NULL		is a target for	NULL	putative			Cdc42	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_35_22537_s_105	9712880	2 Finally, similar to the cytosolic IQGAPs ( 21), binding of Golgi p180 to Cdc42 was competed by the p21-activated kinase, a putative target for Cdc42, but not by the Cdc42-GAP (data not shown).	bind
56900	5	6981	6	10	NULL	0	NULL	p21-activated kinase			is not target for					Cdc42-GAP					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_35_22537_s_105	9712880	2 Finally, similar to the cytosolic IQGAPs ( 21), binding of Golgi p180 to Cdc42 was competed by the p21-activated kinase, a putative target for Cdc42, but not by the Cdc42-GAP (data not shown).	bind
25804	1	6982	5	13	NULL	NULL	NULL	gamma complex	GP		bind					ADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_12_10033_s_196	12519754	2 Following ATP hydrolysis, the ADP-bound form of gamma complex rapidly releases DNA.	bind
25805	2	6982	5	13	NULL	NULL	NULL	statement 1	Process		release		rapidly			DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_12_10033_s_196	12519754	2 Following ATP hydrolysis, the ADP-bound form of gamma complex rapidly releases DNA.	bind
25806	3	6982	5	13	NULL	NULL	NULL	statement 2	Process		occurs following					ATP	Chemical	hydrolysis of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_12_10033_s_196	12519754	2 Following ATP hydrolysis, the ADP-bound form of gamma complex rapidly releases DNA.	bind
21041	1	6982	6	NULL	NULL	0	NULL	ADP	NULL		bind	NULL				gamma complex	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_12_10033_s_196	12519754	2 Following ATP hydrolysis, the ADP-bound form of gamma complex rapidly releases DNA.	bind
21042	2	6982	6	NULL	NULL	0	NULL	statement 1	NULL		releases	NULL	rapidly			DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_12_10033_s_196	12519754	2 Following ATP hydrolysis, the ADP-bound form of gamma complex rapidly releases DNA.	bind
21043	3	6982	6	NULL	NULL	0	NULL	statement 2	NULL		occurs following	NULL				ATP	NULL	hydrolysis of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_12_10033_s_196	12519754	2 Following ATP hydrolysis, the ADP-bound form of gamma complex rapidly releases DNA.	bind
25807	1	6984	5	13	NULL	NULL	NULL	C6PS molecules	Chemical		bind					FVa	GP	bovine			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_33_29765_s_35	12045194	2 Four C6PS molecules also bind to bovine FVa to induce conformational and functional changes ( 10).	bind
25808	2	6984	5	13	NULL	NULL	NULL	statement 1	Process		induces					FVa 	GP	conformational change of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_33_29765_s_35	12045194	2 Four C6PS molecules also bind to bovine FVa to induce conformational and functional changes ( 10).	bind
25809	3	6984	5	13	NULL	NULL	NULL	statement 1	Process		induces					FVa	GP	functional change of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_33_29765_s_35	12045194	2 Four C6PS molecules also bind to bovine FVa to induce conformational and functional changes ( 10).	bind
21044	1	6984	6	NULL	NULL	0	NULL	C6PS molecules	NULL		bind	NULL				FVa	NULL	bovine			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_33_29765_s_35	12045194	2 Four C6PS molecules also bind to bovine FVa to induce conformational and functional changes ( 10).	bind
31181	2	6984	6	NULL	NULL	0	NULL	statement 1	NULL		induces	NULL				FVa	NULL	functional changes of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_33_29765_s_35	12045194	2 Four C6PS molecules also bind to bovine FVa to induce conformational and functional changes ( 10).	bind
31182	3	6984	6	NULL	NULL	0	NULL	statement 1	NULL		induces	NULL				FVa	NULL	conformational changes of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_33_29765_s_35	12045194	2 Four C6PS molecules also bind to bovine FVa to induce conformational and functional changes ( 10).	bind
28991	1	6985	5	13	NULL	NULL	NULL	YAF fraction	GP		is derived from					HeLa cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_49_30880_s_130	9388234	2 Further biochemical analyses have suggested the YAF fraction derived from a variety of cell types ( e.g. HeLa) contains an HMG-I(Y)-like activity as defined by specific interaction with a known IFN-beta HMG-I(Y) DNA-binding site, solubility in 5% perchloric acid, resistance to denaturation and loss of DNA binding activity following exposure to elevated temperature ( e.g. 65  degrees C), and competition of IFN-beta DNA binding activity by poly(dI-dC) DNA and specific alpha-HMG-I antibodies (Fig.  1).	bind
28992	2	6985	5	13	NULL	NULL	NULL	statement 1	GP		contains					HMG-I(Y)-like activity	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_49_30880_s_130	9388234	2 Further biochemical analyses have suggested the YAF fraction derived from a variety of cell types ( e.g. HeLa) contains an HMG-I(Y)-like activity as defined by specific interaction with a known IFN-beta HMG-I(Y) DNA-binding site, solubility in 5% perchloric acid, resistance to denaturation and loss of DNA binding activity following exposure to elevated temperature ( e.g. 65  degrees C), and competition of IFN-beta DNA binding activity by poly(dI-dC) DNA and specific alpha-HMG-I antibodies (Fig.  1).	bind
31526	3	6985	5	13	NULL	NULL	NULL	statement 1	Cell		interacts with		specifically			IFN-beta	GP			HMG-I(Y) DNA-binding site	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_49_30880_s_130	9388234	2 Further biochemical analyses have suggested the YAF fraction derived from a variety of cell types ( e.g. HeLa) contains an HMG-I(Y)-like activity as defined by specific interaction with a known IFN-beta HMG-I(Y) DNA-binding site, solubility in 5% perchloric acid, resistance to denaturation and loss of DNA binding activity following exposure to elevated temperature ( e.g. 65  degrees C), and competition of IFN-beta DNA binding activity by poly(dI-dC) DNA and specific alpha-HMG-I antibodies (Fig.  1).	bind
31527	4	6985	5	13	NULL	NULL	NULL	statement 1	Cell		resistant to					denaturation	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_49_30880_s_130	9388234	2 Further biochemical analyses have suggested the YAF fraction derived from a variety of cell types ( e.g. HeLa) contains an HMG-I(Y)-like activity as defined by specific interaction with a known IFN-beta HMG-I(Y) DNA-binding site, solubility in 5% perchloric acid, resistance to denaturation and loss of DNA binding activity following exposure to elevated temperature ( e.g. 65  degrees C), and competition of IFN-beta DNA binding activity by poly(dI-dC) DNA and specific alpha-HMG-I antibodies (Fig.  1).	bind
31528	5	6985	5	13	NULL	NULL	NULL	statement 1	Process		losses					DNA binding activity	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_49_30880_s_130	9388234	2 Further biochemical analyses have suggested the YAF fraction derived from a variety of cell types ( e.g. HeLa) contains an HMG-I(Y)-like activity as defined by specific interaction with a known IFN-beta HMG-I(Y) DNA-binding site, solubility in 5% perchloric acid, resistance to denaturation and loss of DNA binding activity following exposure to elevated temperature ( e.g. 65  degrees C), and competition of IFN-beta DNA binding activity by poly(dI-dC) DNA and specific alpha-HMG-I antibodies (Fig.  1).	bind
31529	6	6985	5	13	NULL	NULL	NULL	statement 5	Process		occurs following					elevated temperature		exposure to			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_49_30880_s_130	9388234	2 Further biochemical analyses have suggested the YAF fraction derived from a variety of cell types ( e.g. HeLa) contains an HMG-I(Y)-like activity as defined by specific interaction with a known IFN-beta HMG-I(Y) DNA-binding site, solubility in 5% perchloric acid, resistance to denaturation and loss of DNA binding activity following exposure to elevated temperature ( e.g. 65  degrees C), and competition of IFN-beta DNA binding activity by poly(dI-dC) DNA and specific alpha-HMG-I antibodies (Fig.  1).	bind
31531	7	6985	5	13	NULL	NULL	NULL	IFN-beta	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_49_30880_s_130	9388234	2 Further biochemical analyses have suggested the YAF fraction derived from a variety of cell types ( e.g. HeLa) contains an HMG-I(Y)-like activity as defined by specific interaction with a known IFN-beta HMG-I(Y) DNA-binding site, solubility in 5% perchloric acid, resistance to denaturation and loss of DNA binding activity following exposure to elevated temperature ( e.g. 65  degrees C), and competition of IFN-beta DNA binding activity by poly(dI-dC) DNA and specific alpha-HMG-I antibodies (Fig.  1).	bind
31532	8	6985	5	13	NULL	NULL	NULL	poly(dI-dC) DNA	NucleicAcid		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_49_30880_s_130	9388234	2 Further biochemical analyses have suggested the YAF fraction derived from a variety of cell types ( e.g. HeLa) contains an HMG-I(Y)-like activity as defined by specific interaction with a known IFN-beta HMG-I(Y) DNA-binding site, solubility in 5% perchloric acid, resistance to denaturation and loss of DNA binding activity following exposure to elevated temperature ( e.g. 65  degrees C), and competition of IFN-beta DNA binding activity by poly(dI-dC) DNA and specific alpha-HMG-I antibodies (Fig.  1).	bind
56909	9	6985	5	13	NULL	NULL	NULL	alpha-HMG-I antibodies	GP	specific	bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_49_30880_s_130	9388234	2 Further biochemical analyses have suggested the YAF fraction derived from a variety of cell types ( e.g. HeLa) contains an HMG-I(Y)-like activity as defined by specific interaction with a known IFN-beta HMG-I(Y) DNA-binding site, solubility in 5% perchloric acid, resistance to denaturation and loss of DNA binding activity following exposure to elevated temperature ( e.g. 65  degrees C), and competition of IFN-beta DNA binding activity by poly(dI-dC) DNA and specific alpha-HMG-I antibodies (Fig.  1).	bind
56910	10	6985	5	13	NULL	NULL	NULL	statement 8	Process		compete with					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_49_30880_s_130	9388234	2 Further biochemical analyses have suggested the YAF fraction derived from a variety of cell types ( e.g. HeLa) contains an HMG-I(Y)-like activity as defined by specific interaction with a known IFN-beta HMG-I(Y) DNA-binding site, solubility in 5% perchloric acid, resistance to denaturation and loss of DNA binding activity following exposure to elevated temperature ( e.g. 65  degrees C), and competition of IFN-beta DNA binding activity by poly(dI-dC) DNA and specific alpha-HMG-I antibodies (Fig.  1).	bind
56911	11	6985	5	13	NULL	NULL	NULL	statement 9	Process		compete with					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_49_30880_s_130	9388234	2 Further biochemical analyses have suggested the YAF fraction derived from a variety of cell types ( e.g. HeLa) contains an HMG-I(Y)-like activity as defined by specific interaction with a known IFN-beta HMG-I(Y) DNA-binding site, solubility in 5% perchloric acid, resistance to denaturation and loss of DNA binding activity following exposure to elevated temperature ( e.g. 65  degrees C), and competition of IFN-beta DNA binding activity by poly(dI-dC) DNA and specific alpha-HMG-I antibodies (Fig.  1).	bind
56912	12	6985	5	13	NULL	NULL	NULL	YAF fraction	GP		is soluble in					perchloric acid	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_49_30880_s_130	9388234	2 Further biochemical analyses have suggested the YAF fraction derived from a variety of cell types ( e.g. HeLa) contains an HMG-I(Y)-like activity as defined by specific interaction with a known IFN-beta HMG-I(Y) DNA-binding site, solubility in 5% perchloric acid, resistance to denaturation and loss of DNA binding activity following exposure to elevated temperature ( e.g. 65  degrees C), and competition of IFN-beta DNA binding activity by poly(dI-dC) DNA and specific alpha-HMG-I antibodies (Fig.  1).	bind
21230	1	6985	6	NULL	NULL	0	NULL	YAF fractions	NULL		contains	NULL				HMG-I(Y)-like activity	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_49_30880_s_130	9388234	2 Further biochemical analyses have suggested the YAF fraction derived from a variety of cell types ( e.g. HeLa) contains an HMG-I(Y)-like activity as defined by specific interaction with a known IFN-beta HMG-I(Y) DNA-binding site, solubility in 5% perchloric acid, resistance to denaturation and loss of DNA binding activity following exposure to elevated temperature ( e.g. 65  degrees C), and competition of IFN-beta DNA binding activity by poly(dI-dC) DNA and specific alpha-HMG-I antibodies (Fig.  1).	bind
21247	2	6985	6	NULL	NULL	0	NULL	YAF fraction	NULL		bind	NULL				IFN-beta	NULL			HMG-I(Y) DNA-binding site	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_49_30880_s_130	9388234	2 Further biochemical analyses have suggested the YAF fraction derived from a variety of cell types ( e.g. HeLa) contains an HMG-I(Y)-like activity as defined by specific interaction with a known IFN-beta HMG-I(Y) DNA-binding site, solubility in 5% perchloric acid, resistance to denaturation and loss of DNA binding activity following exposure to elevated temperature ( e.g. 65  degrees C), and competition of IFN-beta DNA binding activity by poly(dI-dC) DNA and specific alpha-HMG-I antibodies (Fig.  1).	bind
21248	3	6985	6	NULL	NULL	0	NULL	YAF fraction	NULL		is soluble in	NULL				perchloric acid	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_49_30880_s_130	9388234	2 Further biochemical analyses have suggested the YAF fraction derived from a variety of cell types ( e.g. HeLa) contains an HMG-I(Y)-like activity as defined by specific interaction with a known IFN-beta HMG-I(Y) DNA-binding site, solubility in 5% perchloric acid, resistance to denaturation and loss of DNA binding activity following exposure to elevated temperature ( e.g. 65  degrees C), and competition of IFN-beta DNA binding activity by poly(dI-dC) DNA and specific alpha-HMG-I antibodies (Fig.  1).	bind
21249	4	6985	6	NULL	NULL	0	NULL	YAF fraction	NULL		is resistant to	NULL				denaturation	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_49_30880_s_130	9388234	2 Further biochemical analyses have suggested the YAF fraction derived from a variety of cell types ( e.g. HeLa) contains an HMG-I(Y)-like activity as defined by specific interaction with a known IFN-beta HMG-I(Y) DNA-binding site, solubility in 5% perchloric acid, resistance to denaturation and loss of DNA binding activity following exposure to elevated temperature ( e.g. 65  degrees C), and competition of IFN-beta DNA binding activity by poly(dI-dC) DNA and specific alpha-HMG-I antibodies (Fig.  1).	bind
21250	5	6985	6	10	NULL	0	NULL	YAF fraction			loses					DNA binding activity					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_49_30880_s_130	9388234	2 Further biochemical analyses have suggested the YAF fraction derived from a variety of cell types ( e.g. HeLa) contains an HMG-I(Y)-like activity as defined by specific interaction with a known IFN-beta HMG-I(Y) DNA-binding site, solubility in 5% perchloric acid, resistance to denaturation and loss of DNA binding activity following exposure to elevated temperature ( e.g. 65  degrees C), and competition of IFN-beta DNA binding activity by poly(dI-dC) DNA and specific alpha-HMG-I antibodies (Fig.  1).	bind
21251	6	6985	6	10	NULL	0	NULL	statement 5			upon exposure to					elevated temperature					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_49_30880_s_130	9388234	2 Further biochemical analyses have suggested the YAF fraction derived from a variety of cell types ( e.g. HeLa) contains an HMG-I(Y)-like activity as defined by specific interaction with a known IFN-beta HMG-I(Y) DNA-binding site, solubility in 5% perchloric acid, resistance to denaturation and loss of DNA binding activity following exposure to elevated temperature ( e.g. 65  degrees C), and competition of IFN-beta DNA binding activity by poly(dI-dC) DNA and specific alpha-HMG-I antibodies (Fig.  1).	bind
21253	7	6985	6	10	NULL	0	NULL	 IFN-beta			bind					DNA					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_49_30880_s_130	9388234	2 Further biochemical analyses have suggested the YAF fraction derived from a variety of cell types ( e.g. HeLa) contains an HMG-I(Y)-like activity as defined by specific interaction with a known IFN-beta HMG-I(Y) DNA-binding site, solubility in 5% perchloric acid, resistance to denaturation and loss of DNA binding activity following exposure to elevated temperature ( e.g. 65  degrees C), and competition of IFN-beta DNA binding activity by poly(dI-dC) DNA and specific alpha-HMG-I antibodies (Fig.  1).	bind
56904	8	6985	6	10	NULL	0	NULL	poly(dI-dC) DNA			bind					DNA					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_49_30880_s_130	9388234	2 Further biochemical analyses have suggested the YAF fraction derived from a variety of cell types ( e.g. HeLa) contains an HMG-I(Y)-like activity as defined by specific interaction with a known IFN-beta HMG-I(Y) DNA-binding site, solubility in 5% perchloric acid, resistance to denaturation and loss of DNA binding activity following exposure to elevated temperature ( e.g. 65  degrees C), and competition of IFN-beta DNA binding activity by poly(dI-dC) DNA and specific alpha-HMG-I antibodies (Fig.  1).	bind
56905	9	6985	6	10	NULL	0	NULL	alpha-HMG-I antibodies		specific	bind					DNA					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_49_30880_s_130	9388234	2 Further biochemical analyses have suggested the YAF fraction derived from a variety of cell types ( e.g. HeLa) contains an HMG-I(Y)-like activity as defined by specific interaction with a known IFN-beta HMG-I(Y) DNA-binding site, solubility in 5% perchloric acid, resistance to denaturation and loss of DNA binding activity following exposure to elevated temperature ( e.g. 65  degrees C), and competition of IFN-beta DNA binding activity by poly(dI-dC) DNA and specific alpha-HMG-I antibodies (Fig.  1).	bind
56906	10	6985	6	10	NULL	0	NULL	statement 8			compete with					statement 7					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_49_30880_s_130	9388234	2 Further biochemical analyses have suggested the YAF fraction derived from a variety of cell types ( e.g. HeLa) contains an HMG-I(Y)-like activity as defined by specific interaction with a known IFN-beta HMG-I(Y) DNA-binding site, solubility in 5% perchloric acid, resistance to denaturation and loss of DNA binding activity following exposure to elevated temperature ( e.g. 65  degrees C), and competition of IFN-beta DNA binding activity by poly(dI-dC) DNA and specific alpha-HMG-I antibodies (Fig.  1).	bind
56907	11	6985	6	10	NULL	0	NULL	statement 9			compete with					statement 7					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_49_30880_s_130	9388234	2 Further biochemical analyses have suggested the YAF fraction derived from a variety of cell types ( e.g. HeLa) contains an HMG-I(Y)-like activity as defined by specific interaction with a known IFN-beta HMG-I(Y) DNA-binding site, solubility in 5% perchloric acid, resistance to denaturation and loss of DNA binding activity following exposure to elevated temperature ( e.g. 65  degrees C), and competition of IFN-beta DNA binding activity by poly(dI-dC) DNA and specific alpha-HMG-I antibodies (Fig.  1).	bind
56908	12	6985	6	10	NULL	0	NULL	YAF fraction			derived from					HeLa cells					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_49_30880_s_130	9388234	2 Further biochemical analyses have suggested the YAF fraction derived from a variety of cell types ( e.g. HeLa) contains an HMG-I(Y)-like activity as defined by specific interaction with a known IFN-beta HMG-I(Y) DNA-binding site, solubility in 5% perchloric acid, resistance to denaturation and loss of DNA binding activity following exposure to elevated temperature ( e.g. 65  degrees C), and competition of IFN-beta DNA binding activity by poly(dI-dC) DNA and specific alpha-HMG-I antibodies (Fig.  1).	bind
31521	1	6986	5	13	NULL	NULL	NULL	occludin	GP		bind		may			TJ-scaffolding proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49644_s_203	14512431	2 Further experiments are needed to investigate the regulation and binding affinity between occludin and the different TJ-scaffolding proteins.	bind
21048	1	6986	6	NULL	NULL	0	NULL	occludin	NULL		bind	NULL	may			TJ-scaffolding proteins	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49644_s_203	14512431	2 Further experiments are needed to investigate the regulation and binding affinity between occludin and the different TJ-scaffolding proteins.	bind
31522	1	6987	5	13	NULL	NULL	NULL	FRP/Frzb	GP		bind					Wnt	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_27_19465_s_280	10383463	2 Further studies will be required to determine whether Sk/Dkk binds Wnt, like FRP/Frzb and Cerberus, or antagonizes Wnt signaling indirectly through an independent inhibitory pathway.	bind
31523	2	6987	5	13	NULL	NULL	NULL	Cerberus	GP		bind					Wnt	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_27_19465_s_280	10383463	2 Further studies will be required to determine whether Sk/Dkk binds Wnt, like FRP/Frzb and Cerberus, or antagonizes Wnt signaling indirectly through an independent inhibitory pathway.	bind
21049	1	6987	6	NULL	NULL	0	NULL	FRP/Frzb	NULL		bind	NULL				Wnt	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_27_19465_s_280	10383463	2 Further studies will be required to determine whether Sk/Dkk binds Wnt, like FRP/Frzb and Cerberus, or antagonizes Wnt signaling indirectly through an independent inhibitory pathway.	bind
21050	2	6987	6	NULL	NULL	0	NULL	Cerberus	NULL		bind	NULL				Wnt	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_27_19465_s_280	10383463	2 Further studies will be required to determine whether Sk/Dkk binds Wnt, like FRP/Frzb and Cerberus, or antagonizes Wnt signaling indirectly through an independent inhibitory pathway.	bind
25810	1	6988	5	13	NULL	NULL	NULL	ProRS	GP	archaeal-type T. thermophilus	bind					cysteine	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_38_34749_s_177	12130658	2 Further support is derived from suggestions based on a modeling experiment that the archaeal-type  T. thermophilus ProRS could also bind cysteine ( 35).	bind
21109	1	6988	6	NULL	NULL	0	NULL	 ProRS	NULL	archaeal-type T. thermophilus	bind	NULL				cysteine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_38_34749_s_177	12130658	2 Further support is derived from suggestions based on a modeling experiment that the archaeal-type  T. thermophilus ProRS could also bind cysteine ( 35).	bind
25811	1	6989	5	13	NULL	NULL	NULL	p68	GP		bind					p180	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_23_20541_s_184	11927598	2 Furthermore, binding of p68 to p180 induces a conformational change in the latter polypeptide ( 51).	bind
25812	2	6989	5	13	NULL	NULL	NULL	statement 1	Process		induces					p180	GP	conformational change in			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_23_20541_s_184	11927598	2 Furthermore, binding of p68 to p180 induces a conformational change in the latter polypeptide ( 51).	bind
21128	1	6989	6	NULL	NULL	0	NULL	p68	NULL		bind	NULL				p180	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_23_20541_s_184	11927598	2 Furthermore, binding of p68 to p180 induces a conformational change in the latter polypeptide ( 51).	bind
21160	2	6989	6	NULL	NULL	0	NULL	statement 1	NULL		induce	NULL				p180	NULL	conformational change of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_23_20541_s_184	11927598	2 Furthermore, binding of p68 to p180 induces a conformational change in the latter polypeptide ( 51).	bind
25813	1	6990	5	13	NULL	NULL	NULL	PAI-1	GP		does not bind								heparin-binding domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_5112_s_220	9030577	2 Furthermore, these data indicate that PAI-1 does not bind to the heparin-binding domain, as that would alter the quenching behavior of the coumarin probe.	bind
25814	2	6990	5	13	NULL	NULL	NULL				alter			heparin-binding domain		coumarin probe	NucleicAcid	quenching behaviour of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_5112_s_220	9030577	2 Furthermore, these data indicate that PAI-1 does not bind to the heparin-binding domain, as that would alter the quenching behavior of the coumarin probe.	bind
58593	3	6990	5	13	NULL	NULL	NULL	statement 1	Process		does not alter					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_5112_s_220	9030577	2 Furthermore, these data indicate that PAI-1 does not bind to the heparin-binding domain, as that would alter the quenching behavior of the coumarin probe.	bind
21161	1	6990	6	NULL	NULL	0	NULL	PAI-1	NULL		does not bind	NULL					NULL		heparin binding domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_8_5112_s_220	9030577	2 Furthermore, these data indicate that PAI-1 does not bind to the heparin-binding domain, as that would alter the quenching behavior of the coumarin probe.	bind
21162	2	6990	6	10	NULL	0	NULL				alter			heparin-binding domain		coumarin probe		quenching behavior of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_5112_s_220	9030577	2 Furthermore, these data indicate that PAI-1 does not bind to the heparin-binding domain, as that would alter the quenching behavior of the coumarin probe.	bind
21163	3	6990	6	NULL	NULL	0	NULL	statement 1	NULL		does not alter	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_8_5112_s_220	9030577	2 Furthermore, these data indicate that PAI-1 does not bind to the heparin-binding domain, as that would alter the quenching behavior of the coumarin probe.	bind
25815	1	6991	5	13	NULL	NULL	NULL	E2	GP		bind					RSP5	GP	S. cerevisiae			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_21_13548_s_52	9153201	2 Furthermore, we show that a different subfamily of structurally related E2s bind to the  S. cerevisiae Hect protein RSP5 ( 17,  23).	bind
25816	2	6991	5	13	NULL	NULL	NULL	RSP5	GP		is a type of					Hect protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_21_13548_s_52	9153201	2 Furthermore, we show that a different subfamily of structurally related E2s bind to the  S. cerevisiae Hect protein RSP5 ( 17,  23).	bind
21164	1	6991	6	10	NULL	0	NULL	E2	NULL		bind	NULL				RSP5	NULL	S. cerevisiae 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_21_13548_s_52	9153201	2 Furthermore, we show that a different subfamily of structurally related E2s bind to the  S. cerevisiae Hect protein RSP5 ( 17,  23).	bind
44822	2	6991	6	10	NULL	0	NULL	RSP5	NULL		is a type of	NULL				hect protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_21_13548_s_52	9153201	2 Furthermore, we show that a different subfamily of structurally related E2s bind to the  S. cerevisiae Hect protein RSP5 ( 17,  23).	bind
25817	1	6992	5	13	NULL	NULL	NULL	GCK	GP		associates with					TRAF6.3	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_9_5259_s_135	10026130	2 GCK can also associate  in vivo with TRAF6.3 The CT extensions (Fig.  1) are required for the binding of GCK and GCKR to TRAF2 ( 46).	bind
25818	2	6992	5	13	NULL	NULL	NULL	GCK	GP		bind					TRAF2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_9_5259_s_135	10026130	2 GCK can also associate  in vivo with TRAF6.3 The CT extensions (Fig.  1) are required for the binding of GCK and GCKR to TRAF2 ( 46).	bind
25819	3	6992	5	13	NULL	NULL	NULL				is required for			CT extensions		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_9_5259_s_135	10026130	2 GCK can also associate  in vivo with TRAF6.3 The CT extensions (Fig.  1) are required for the binding of GCK and GCKR to TRAF2 ( 46).	bind
25820	4	6992	5	13	NULL	NULL	NULL	GCKR	GP		bind					TRAF2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_9_5259_s_135	10026130	2 GCK can also associate  in vivo with TRAF6.3 The CT extensions (Fig.  1) are required for the binding of GCK and GCKR to TRAF2 ( 46).	bind
25821	5	6992	5	13	NULL	NULL	NULL				is required for			CT extensions		statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_9_5259_s_135	10026130	2 GCK can also associate  in vivo with TRAF6.3 The CT extensions (Fig.  1) are required for the binding of GCK and GCKR to TRAF2 ( 46).	bind
21165	1	6992	6	NULL	NULL	0	NULL	GCK	NULL		associate	NULL				TRAF6.3	NULL				NULL	in vivo	0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5259_s_135	10026130	2 GCK can also associate  in vivo with TRAF6.3 The CT extensions (Fig.  1) are required for the binding of GCK and GCKR to TRAF2 ( 46).	bind
21166	2	6992	6	10	NULL	0	NULL	GCK			bind					TRAF2					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_9_5259_s_135	10026130	2 GCK can also associate  in vivo with TRAF6.3 The CT extensions (Fig.  1) are required for the binding of GCK and GCKR to TRAF2 ( 46).	bind
21167	3	6992	6	10	NULL	0	NULL	GCKR			bind					TRAF2					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_9_5259_s_135	10026130	2 GCK can also associate  in vivo with TRAF6.3 The CT extensions (Fig.  1) are required for the binding of GCK and GCKR to TRAF2 ( 46).	bind
21168	4	6992	6	NULL	NULL	0	NULL	statement 2	NULL		requires	NULL					NULL		CT extensions		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5259_s_135	10026130	2 GCK can also associate  in vivo with TRAF6.3 The CT extensions (Fig.  1) are required for the binding of GCK and GCKR to TRAF2 ( 46).	bind
21169	5	6992	6	NULL	NULL	0	NULL	statement 3	NULL		requires	NULL					NULL		CT extensions		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5259_s_135	10026130	2 GCK can also associate  in vivo with TRAF6.3 The CT extensions (Fig.  1) are required for the binding of GCK and GCKR to TRAF2 ( 46).	bind
25822	1	6993	5	13	NULL	NULL	NULL	capping enzyme	GP	mammalian	bind			triphosphatase domain		Spt5	GP	mammalian			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_22_19639_s_334	11893740	2 Given that the individual triphosphatase and guanylyltransferase domains of mammalian capping enzyme bind  in vitro to mammalian Spt5 ( 13), our results suggest that the structural basis for the Spt5-capping enzyme interaction is distinct in fission yeast  versus mammals.	bind
25824	2	6993	5	13	NULL	NULL	NULL	capping enzyme	GP	mammalian	bind			guanylyltransferase domain		Spt5	GP	mammalian			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_22_19639_s_334	11893740	2 Given that the individual triphosphatase and guanylyltransferase domains of mammalian capping enzyme bind  in vitro to mammalian Spt5 ( 13), our results suggest that the structural basis for the Spt5-capping enzyme interaction is distinct in fission yeast  versus mammals.	bind
25825	3	6993	5	13	NULL	NULL	NULL	Spt5	GP	fission yeast	bind					capping enzyme	GP	fission yeast			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_22_19639_s_334	11893740	2 Given that the individual triphosphatase and guanylyltransferase domains of mammalian capping enzyme bind  in vitro to mammalian Spt5 ( 13), our results suggest that the structural basis for the Spt5-capping enzyme interaction is distinct in fission yeast  versus mammals.	bind
21170	1	6993	6	NULL	NULL	0	NULL	capping enzyme	NULL	mammalian	bind	NULL		triphosphatase domain		Spt5	NULL	mammalian			NULL	in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_277_22_19639_s_334	11893740	2 Given that the individual triphosphatase and guanylyltransferase domains of mammalian capping enzyme bind  in vitro to mammalian Spt5 ( 13), our results suggest that the structural basis for the Spt5-capping enzyme interaction is distinct in fission yeast  versus mammals.	bind
21171	2	6993	6	NULL	NULL	0	NULL	capping enzyme	NULL	mammalian	bind	NULL		guanylyltransferase domain		Spt5	NULL	mammalian			NULL	in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_277_22_19639_s_334	11893740	2 Given that the individual triphosphatase and guanylyltransferase domains of mammalian capping enzyme bind  in vitro to mammalian Spt5 ( 13), our results suggest that the structural basis for the Spt5-capping enzyme interaction is distinct in fission yeast  versus mammals.	bind
44846	3	6993	6	10	NULL	0	NULL	Spt5	NULL	fission yeast	bind	NULL				capping enzyme	NULL	fission yeast			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_22_19639_s_334	11893740	2 Given that the individual triphosphatase and guanylyltransferase domains of mammalian capping enzyme bind  in vitro to mammalian Spt5 ( 13), our results suggest that the structural basis for the Spt5-capping enzyme interaction is distinct in fission yeast  versus mammals.	bind
25828	1	6994	5	13	NULL	NULL	NULL	snRNP	GP		bind					pre-mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17333_s_276	9211871	2 Given the known order of snRNP binding to the pre-mRNA during spliceosome assembly (for reviews, see Refs.	bind
25829	2	6994	5	13	NULL	NULL	NULL	statement 1	Process		occurs during					spliceosome		assembly of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17333_s_276	9211871	2 Given the known order of snRNP binding to the pre-mRNA during spliceosome assembly (for reviews, see Refs.	bind
21172	1	6994	6	NULL	NULL	0	NULL	snRNP	NULL		bind	NULL				pre-mRNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_28_17333_s_276	9211871	2 Given the known order of snRNP binding to the pre-mRNA during spliceosome assembly (for reviews, see Refs.	bind
21173	2	6994	6	10	NULL	0	NULL	statement 1			occurs during					spliceosome 		assembly of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17333_s_276	9211871	2 Given the known order of snRNP binding to the pre-mRNA during spliceosome assembly (for reviews, see Refs.	bind
25830	1	6995	5	13	NULL	NULL	NULL	ERp57	GP		bind		non-specifically			CRT	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_33_29686_s_310	12052826	2 Given these solubility changes, we considered the possibility that Zn2+-dependent ERp57 binding to CRT and CNX is nonspecific.	bind
25831	2	6995	5	13	NULL	NULL	NULL	statement 1	Process		is dependent on					Zn2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_33_29686_s_310	12052826	2 Given these solubility changes, we considered the possibility that Zn2+-dependent ERp57 binding to CRT and CNX is nonspecific.	bind
25833	3	6995	5	13	NULL	NULL	NULL	ERp57	GP		bind		non-specifically			CNX	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_33_29686_s_310	12052826	2 Given these solubility changes, we considered the possibility that Zn2+-dependent ERp57 binding to CRT and CNX is nonspecific.	bind
25834	4	6995	5	13	NULL	NULL	NULL	statement 3	Process		is dependent on					Zn2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_33_29686_s_310	12052826	2 Given these solubility changes, we considered the possibility that Zn2+-dependent ERp57 binding to CRT and CNX is nonspecific.	bind
21174	1	6995	6	NULL	NULL	0	NULL	ERp57	NULL		bind	NULL	non-specifically			CRT	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_33_29686_s_310	12052826	2 Given these solubility changes, we considered the possibility that Zn2+-dependent ERp57 binding to CRT and CNX is nonspecific.	bind
21175	2	6995	6	NULL	NULL	0	NULL	ERp57	NULL		bind	NULL	non-specifically			CNX	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_33_29686_s_310	12052826	2 Given these solubility changes, we considered the possibility that Zn2+-dependent ERp57 binding to CRT and CNX is nonspecific.	bind
21176	3	6995	6	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				Zn2+	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_33_29686_s_310	12052826	2 Given these solubility changes, we considered the possibility that Zn2+-dependent ERp57 binding to CRT and CNX is nonspecific.	bind
21177	4	6995	6	NULL	NULL	0	NULL	statement 2	NULL		is dependent on	NULL				Zn2+	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_33_29686_s_310	12052826	2 Given these solubility changes, we considered the possibility that Zn2+-dependent ERp57 binding to CRT and CNX is nonspecific.	bind
26407	1	6996	5	13	NULL	NULL	NULL	ROKalpha binding domain antibody	GP		activates					ROKalpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_12680_s_173	11815607	2 h after incubation with the individual antibodies, the filter was subjected to RhoA binding with GST-RhoAV14 loaded with [gamma-32]GTP before exposing to x-ray film for 2 h.  B, ROKalpha binding domain antibody activates ROKalpha.	bind
21178	1	6996	6	NULL	NULL	0	NULL	antiROKalpha binding domain antibody	NULL		activates	NULL				ROKalpha	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_12680_s_173	11815607	2 h after incubation with the individual antibodies, the filter was subjected to RhoA binding with GST-RhoAV14 loaded with [gamma-32]GTP before exposing to x-ray film for 2 h.  B, ROKalpha binding domain antibody activates ROKalpha.	bind
26408	1	6997	5	13	NULL	NULL	NULL	heparin	Chemical		bind					BPIs	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2149_s_128	8999916	2 Heparin Binding of the BPIs, LBPs, and Fusion Proteins Is Dependent on the N-terminal LPS Binding Domain	bind
26409	2	6997	5	13	NULL	NULL	NULL	statement 1	Process		is dependent on								N-terminal LPS binding domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2149_s_128	8999916	2 Heparin Binding of the BPIs, LBPs, and Fusion Proteins Is Dependent on the N-terminal LPS Binding Domain	bind
26410	3	6997	5	13	NULL	NULL	NULL	heparin	Chemical		bind					LBPs	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2149_s_128	8999916	2 Heparin Binding of the BPIs, LBPs, and Fusion Proteins Is Dependent on the N-terminal LPS Binding Domain	bind
26411	4	6997	5	13	NULL	NULL	NULL	statement 3	Process		is dependent on								N-terminal LPS binding domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2149_s_128	8999916	2 Heparin Binding of the BPIs, LBPs, and Fusion Proteins Is Dependent on the N-terminal LPS Binding Domain	bind
21179	1	6997	6	NULL	NULL	0	NULL	Heparin	NULL		bind	NULL				BPIs	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_4_2149_s_128	8999916	2 Heparin Binding of the BPIs, LBPs, and Fusion Proteins Is Dependent on the N-terminal LPS Binding Domain	bind
21180	2	6997	6	NULL	NULL	0	NULL	heparin	NULL		bind	NULL				LBPs	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_4_2149_s_128	8999916	2 Heparin Binding of the BPIs, LBPs, and Fusion Proteins Is Dependent on the N-terminal LPS Binding Domain	bind
21182	3	6997	6	10	NULL	0	NULL	statement 1			is dependent on								N-terminal LPS Binding Domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2149_s_128	8999916	2 Heparin Binding of the BPIs, LBPs, and Fusion Proteins Is Dependent on the N-terminal LPS Binding Domain	bind
21183	4	6997	6	10	NULL	0	NULL	statement 2			is dependent on								N-terminal LPS Binding Domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2149_s_128	8999916	2 Heparin Binding of the BPIs, LBPs, and Fusion Proteins Is Dependent on the N-terminal LPS Binding Domain	bind
26412	1	6999	5	13	NULL	NULL	NULL	TSP2	GP		bind					pro-MMP2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_11_8403_s_95	11113133	2 However, as revealed by a gelatinolytic assay with soluble [3]gelatin as a substrate, the binding of TSP2 to pro-MMP2 did not inhibit its activation by APMA (Fig.  2).	bind
26413	2	6999	5	13	NULL	NULL	NULL	pro-MMP2	GP		is activated by					APMA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_11_8403_s_95	11113133	2 However, as revealed by a gelatinolytic assay with soluble [3]gelatin as a substrate, the binding of TSP2 to pro-MMP2 did not inhibit its activation by APMA (Fig.  2).	bind
26414	3	6999	5	13	NULL	NULL	NULL	statement 1	Process		does not inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_11_8403_s_95	11113133	2 However, as revealed by a gelatinolytic assay with soluble [3]gelatin as a substrate, the binding of TSP2 to pro-MMP2 did not inhibit its activation by APMA (Fig.  2).	bind
21259	1	6999	6	NULL	NULL	0	NULL	TSP2	NULL		bind	NULL				pro-MMP2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_11_8403_s_95	11113133	2 However, as revealed by a gelatinolytic assay with soluble [3]gelatin as a substrate, the binding of TSP2 to pro-MMP2 did not inhibit its activation by APMA (Fig.  2).	bind
21260	2	6999	6	10	NULL	0	NULL	APMA			activates					pro-MMP2					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_11_8403_s_95	11113133	2 However, as revealed by a gelatinolytic assay with soluble [3]gelatin as a substrate, the binding of TSP2 to pro-MMP2 did not inhibit its activation by APMA (Fig.  2).	bind
21261	3	6999	6	10	NULL	0	NULL	statement 1			does not inhibit					statement 2					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_11_8403_s_95	11113133	2 However, as revealed by a gelatinolytic assay with soluble [3]gelatin as a substrate, the binding of TSP2 to pro-MMP2 did not inhibit its activation by APMA (Fig.  2).	bind
26415	1	7000	5	13	NULL	NULL	NULL	MDM2	GP		inhibit					MyoD	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_25_22615_s_113	12702724	2 However, because the region of MDM2 that inhibits MyoD  binds to both Sp1 and pRb ( ),  these observations suggest that pRb and/or Sp1 were potential targets for MDM2  inhibition.	bind
26416	2	7000	5	13	NULL	NULL	NULL	MDM2	GP		bind					Sp1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_25_22615_s_113	12702724	2 However, because the region of MDM2 that inhibits MyoD  binds to both Sp1 and pRb ( ),  these observations suggest that pRb and/or Sp1 were potential targets for MDM2  inhibition.	bind
26417	3	7000	5	13	NULL	NULL	NULL	MDM2	GP		bind					pRb	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_25_22615_s_113	12702724	2 However, because the region of MDM2 that inhibits MyoD  binds to both Sp1 and pRb ( ),  these observations suggest that pRb and/or Sp1 were potential targets for MDM2  inhibition.	bind
26418	4	7000	5	13	NULL	NULL	NULL	MDM2	GP		target for		potentially			pRb	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_25_22615_s_113	12702724	2 However, because the region of MDM2 that inhibits MyoD  binds to both Sp1 and pRb ( ),  these observations suggest that pRb and/or Sp1 were potential targets for MDM2  inhibition.	bind
26419	5	7000	5	13	NULL	NULL	NULL	MDM2	GP		target for		potentially			Sp1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_25_22615_s_113	12702724	2 However, because the region of MDM2 that inhibits MyoD  binds to both Sp1 and pRb ( ),  these observations suggest that pRb and/or Sp1 were potential targets for MDM2  inhibition.	bind
31524	6	7000	5	13	NULL	NULL	NULL	statement 4	Process		inhibits					pRb	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_25_22615_s_113	12702724	2 However, because the region of MDM2 that inhibits MyoD  binds to both Sp1 and pRb ( ),  these observations suggest that pRb and/or Sp1 were potential targets for MDM2  inhibition.	bind
31525	7	7000	5	13	NULL	NULL	NULL	statement 5	Process		inhibits					Sp1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_25_22615_s_113	12702724	2 However, because the region of MDM2 that inhibits MyoD  binds to both Sp1 and pRb ( ),  these observations suggest that pRb and/or Sp1 were potential targets for MDM2  inhibition.	bind
21262	1	7000	6	NULL	NULL	0	NULL	MDM2	NULL		inhibits	NULL				MyoD	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_25_22615_s_113	12702724	2 However, because the region of MDM2 that inhibits MyoD  binds to both Sp1 and pRb ( ),  these observations suggest that pRb and/or Sp1 were potential targets for MDM2  inhibition.	bind
21263	2	7000	6	NULL	NULL	0	NULL	MDM2	NULL		bind	NULL				Sp1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_25_22615_s_113	12702724	2 However, because the region of MDM2 that inhibits MyoD  binds to both Sp1 and pRb ( ),  these observations suggest that pRb and/or Sp1 were potential targets for MDM2  inhibition.	bind
21264	3	7000	6	NULL	NULL	0	NULL	MDM2	NULL		bind	NULL				pRb	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_25_22615_s_113	12702724	2 However, because the region of MDM2 that inhibits MyoD  binds to both Sp1 and pRb ( ),  these observations suggest that pRb and/or Sp1 were potential targets for MDM2  inhibition.	bind
21265	4	7000	6	NULL	NULL	0	NULL	MDM2	NULL		target for	NULL	potentially			pRb	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_25_22615_s_113	12702724	2 However, because the region of MDM2 that inhibits MyoD  binds to both Sp1 and pRb ( ),  these observations suggest that pRb and/or Sp1 were potential targets for MDM2  inhibition.	bind
21266	5	7000	6	NULL	NULL	0	NULL	statement 4	NULL		inhibit	NULL				pRb	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_25_22615_s_113	12702724	2 However, because the region of MDM2 that inhibits MyoD  binds to both Sp1 and pRb ( ),  these observations suggest that pRb and/or Sp1 were potential targets for MDM2  inhibition.	bind
30720	6	7000	6	NULL	NULL	0	NULL	MDM2	NULL		target for	NULL	potentially			Sp1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_25_22615_s_113	12702724	2 However, because the region of MDM2 that inhibits MyoD  binds to both Sp1 and pRb ( ),  these observations suggest that pRb and/or Sp1 were potential targets for MDM2  inhibition.	bind
30721	7	7000	6	NULL	NULL	0	NULL	statement 6	NULL		inhibits	NULL				Sp1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_25_22615_s_113	12702724	2 However, because the region of MDM2 that inhibits MyoD  binds to both Sp1 and pRb ( ),  these observations suggest that pRb and/or Sp1 were potential targets for MDM2  inhibition.	bind
25374	1	7001	7	13	NULL	NULL	NULL	MDM2	GP		binds					Sp1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_25_22615_s_113	12702724	2 However, because the region of MDM2 that inhibits MyoD  binds to both Sp1 and pRb ( 2),  these observations suggest that pRb and/or Sp1 were potential targets for MDM2  inhibition.	bind
25375	2	7001	7	13	NULL	NULL	NULL	MDM2	GP		binds					pRb	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_25_22615_s_113	12702724	2 However, because the region of MDM2 that inhibits MyoD  binds to both Sp1 and pRb ( 2),  these observations suggest that pRb and/or Sp1 were potential targets for MDM2  inhibition.	bind
25376	3	7001	7	13	NULL	NULL	NULL	MDM2	GP		inhibits					MyoD	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_25_22615_s_113	12702724	2 However, because the region of MDM2 that inhibits MyoD  binds to both Sp1 and pRb ( 2),  these observations suggest that pRb and/or Sp1 were potential targets for MDM2  inhibition.	bind
25377	4	7001	7	13	NULL	NULL	NULL	MDM2	GP		target for		potentially			pRb	GP	 inhibition of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_25_22615_s_113	12702724	2 However, because the region of MDM2 that inhibits MyoD  binds to both Sp1 and pRb ( 2),  these observations suggest that pRb and/or Sp1 were potential targets for MDM2  inhibition.	bind
25378	5	7001	7	13	NULL	NULL	NULL	MDM2	GP		target for		potentially			Sp1	GP	inhibition of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_25_22615_s_113	12702724	2 However, because the region of MDM2 that inhibits MyoD  binds to both Sp1 and pRb ( 2),  these observations suggest that pRb and/or Sp1 were potential targets for MDM2  inhibition.	bind
53255	6	7001	7	13	NULL	NULL	NULL	statement 4	Process		inhibits					pRb	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_25_22615_s_113	12702724	2 However, because the region of MDM2 that inhibits MyoD  binds to both Sp1 and pRb ( 2),  these observations suggest that pRb and/or Sp1 were potential targets for MDM2  inhibition.	bind
53256	7	7001	7	13	NULL	NULL	NULL	statement 5	Process		inhibits					Sp1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_25_22615_s_113	12702724	2 However, because the region of MDM2 that inhibits MyoD  binds to both Sp1 and pRb ( 2),  these observations suggest that pRb and/or Sp1 were potential targets for MDM2  inhibition.	bind
22160	1	7003	6	13	NULL	NULL	NULL	DNA-PK	GP		phosphorylates					Ku	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_12_7848_s_274	10075677	2 However, Ku cannot be ruled out as a key target of p460 for its entry into DNA since (i) the consequence on IR sensitivity of mutations in Ku80 DNA-PK phosphorylation sites has not been evaluated yet, (ii) the intrinsic Ku DNA-dependent ATPase activity has been reported to be greatly stimulated when Ku was phosphorylated by DNA-PK ( 23), which could in turn modify its putative helicase activity, (iii) Ku molecules bound to a DNA-PK activating DNA fragment are indeed in a phosphorylated form under kinase permissive conditions.	bind
22162	3	7003	6	13	NULL	NULL	NULL	Ku	GP	ATPase activity of	is dependent on					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_12_7848_s_274	10075677	2 However, Ku cannot be ruled out as a key target of p460 for its entry into DNA since (i) the consequence on IR sensitivity of mutations in Ku80 DNA-PK phosphorylation sites has not been evaluated yet, (ii) the intrinsic Ku DNA-dependent ATPase activity has been reported to be greatly stimulated when Ku was phosphorylated by DNA-PK ( 23), which could in turn modify its putative helicase activity, (iii) Ku molecules bound to a DNA-PK activating DNA fragment are indeed in a phosphorylated form under kinase permissive conditions.	bind
22163	4	7003	6	13	NULL	NULL	NULL	statement 1	Process		stimulates					Ku	GP	intrinsic;;ATPase activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_12_7848_s_274	10075677	2 However, Ku cannot be ruled out as a key target of p460 for its entry into DNA since (i) the consequence on IR sensitivity of mutations in Ku80 DNA-PK phosphorylation sites has not been evaluated yet, (ii) the intrinsic Ku DNA-dependent ATPase activity has been reported to be greatly stimulated when Ku was phosphorylated by DNA-PK ( 23), which could in turn modify its putative helicase activity, (iii) Ku molecules bound to a DNA-PK activating DNA fragment are indeed in a phosphorylated form under kinase permissive conditions.	bind
22165	6	7003	6	13	NULL	NULL	NULL	statement 1	Process		modifies					Ku	GP	putative;;helicase activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_12_7848_s_274	10075677	2 However, Ku cannot be ruled out as a key target of p460 for its entry into DNA since (i) the consequence on IR sensitivity of mutations in Ku80 DNA-PK phosphorylation sites has not been evaluated yet, (ii) the intrinsic Ku DNA-dependent ATPase activity has been reported to be greatly stimulated when Ku was phosphorylated by DNA-PK ( 23), which could in turn modify its putative helicase activity, (iii) Ku molecules bound to a DNA-PK activating DNA fragment are indeed in a phosphorylated form under kinase permissive conditions.	bind
22166	7	7003	6	13	NULL	NULL	NULL	Ku molecules	GP	phosphorylated	bind					DNA-PK	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_12_7848_s_274	10075677	2 However, Ku cannot be ruled out as a key target of p460 for its entry into DNA since (i) the consequence on IR sensitivity of mutations in Ku80 DNA-PK phosphorylation sites has not been evaluated yet, (ii) the intrinsic Ku DNA-dependent ATPase activity has been reported to be greatly stimulated when Ku was phosphorylated by DNA-PK ( 23), which could in turn modify its putative helicase activity, (iii) Ku molecules bound to a DNA-PK activating DNA fragment are indeed in a phosphorylated form under kinase permissive conditions.	bind
22167	8	7003	6	13	NULL	NULL	NULL	statement 7	Process		activates					DNA fragment	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_12_7848_s_274	10075677	2 However, Ku cannot be ruled out as a key target of p460 for its entry into DNA since (i) the consequence on IR sensitivity of mutations in Ku80 DNA-PK phosphorylation sites has not been evaluated yet, (ii) the intrinsic Ku DNA-dependent ATPase activity has been reported to be greatly stimulated when Ku was phosphorylated by DNA-PK ( 23), which could in turn modify its putative helicase activity, (iii) Ku molecules bound to a DNA-PK activating DNA fragment are indeed in a phosphorylated form under kinase permissive conditions.	bind
25379	1	7003	7	NULL	NULL	0	NULL	DNA-PK 	NULL		phosphorylate	NULL				Ku	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_12_7848_s_274	10075677	2 However, Ku cannot be ruled out as a key target of p460 for its entry into DNA since (i) the consequence on IR sensitivity of mutations in Ku80 DNA-PK phosphorylation sites has not been evaluated yet, (ii) the intrinsic Ku DNA-dependent ATPase activity has been reported to be greatly stimulated when Ku was phosphorylated by DNA-PK ( 23), which could in turn modify its putative helicase activity, (iii) Ku molecules bound to a DNA-PK activating DNA fragment are indeed in a phosphorylated form under kinase permissive conditions.	bind
25380	2	7003	7	10	NULL	0	NULL	statement 1	NULL		stimulates	NULL				Ku	NULL	intrinsic;;ATPase activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_12_7848_s_274	10075677	2 However, Ku cannot be ruled out as a key target of p460 for its entry into DNA since (i) the consequence on IR sensitivity of mutations in Ku80 DNA-PK phosphorylation sites has not been evaluated yet, (ii) the intrinsic Ku DNA-dependent ATPase activity has been reported to be greatly stimulated when Ku was phosphorylated by DNA-PK ( 23), which could in turn modify its putative helicase activity, (iii) Ku molecules bound to a DNA-PK activating DNA fragment are indeed in a phosphorylated form under kinase permissive conditions.	bind
25381	4	7003	7	10	NULL	0	NULL	statement 1	NULL		modifies	NULL				Ku	NULL	putative;;helicase activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_12_7848_s_274	10075677	2 However, Ku cannot be ruled out as a key target of p460 for its entry into DNA since (i) the consequence on IR sensitivity of mutations in Ku80 DNA-PK phosphorylation sites has not been evaluated yet, (ii) the intrinsic Ku DNA-dependent ATPase activity has been reported to be greatly stimulated when Ku was phosphorylated by DNA-PK ( 23), which could in turn modify its putative helicase activity, (iii) Ku molecules bound to a DNA-PK activating DNA fragment are indeed in a phosphorylated form under kinase permissive conditions.	bind
25382	5	7003	7	10	NULL	0	NULL	Ku molecules	NULL	phosphorylated	bind	NULL				DNA-PK	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_12_7848_s_274	10075677	2 However, Ku cannot be ruled out as a key target of p460 for its entry into DNA since (i) the consequence on IR sensitivity of mutations in Ku80 DNA-PK phosphorylation sites has not been evaluated yet, (ii) the intrinsic Ku DNA-dependent ATPase activity has been reported to be greatly stimulated when Ku was phosphorylated by DNA-PK ( 23), which could in turn modify its putative helicase activity, (iii) Ku molecules bound to a DNA-PK activating DNA fragment are indeed in a phosphorylated form under kinase permissive conditions.	bind
25383	7	7003	7	10	NULL	0	NULL	statement 5	NULL		occurs under	NULL				kinase permissive condition	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_12_7848_s_274	10075677	2 However, Ku cannot be ruled out as a key target of p460 for its entry into DNA since (i) the consequence on IR sensitivity of mutations in Ku80 DNA-PK phosphorylation sites has not been evaluated yet, (ii) the intrinsic Ku DNA-dependent ATPase activity has been reported to be greatly stimulated when Ku was phosphorylated by DNA-PK ( 23), which could in turn modify its putative helicase activity, (iii) Ku molecules bound to a DNA-PK activating DNA fragment are indeed in a phosphorylated form under kinase permissive conditions.	bind
46413	6	7003	7	10	NULL	0	NULL	statement 5	NULL		activates	NULL				DNA fragment	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_12_7848_s_274	10075677	2 However, Ku cannot be ruled out as a key target of p460 for its entry into DNA since (i) the consequence on IR sensitivity of mutations in Ku80 DNA-PK phosphorylation sites has not been evaluated yet, (ii) the intrinsic Ku DNA-dependent ATPase activity has been reported to be greatly stimulated when Ku was phosphorylated by DNA-PK ( 23), which could in turn modify its putative helicase activity, (iii) Ku molecules bound to a DNA-PK activating DNA fragment are indeed in a phosphorylated form under kinase permissive conditions.	bind
53257	8	7003	7	10	NULL	0	NULL	Ku	NULL	ATPase activity of	is dependent on	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_12_7848_s_274	10075677	2 However, Ku cannot be ruled out as a key target of p460 for its entry into DNA since (i) the consequence on IR sensitivity of mutations in Ku80 DNA-PK phosphorylation sites has not been evaluated yet, (ii) the intrinsic Ku DNA-dependent ATPase activity has been reported to be greatly stimulated when Ku was phosphorylated by DNA-PK ( 23), which could in turn modify its putative helicase activity, (iii) Ku molecules bound to a DNA-PK activating DNA fragment are indeed in a phosphorylated form under kinase permissive conditions.	bind
21267	1	7004	6	13	NULL	NULL	NULL	Ku	GP		bind									C3H-NRE1 microcircles	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_9_5647_s_112	9038175	2 However, over several repetitions of the binding assay, Ku binding to C3H-NRE1 microcircles was consistently about 4-fold lower than binding to the GR-NRE1 microcircles.	bind
21268	2	7004	6	13	NULL	NULL	NULL	Ku	GP		bind									GR-NRE1 microcircles	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_9_5647_s_112	9038175	2 However, over several repetitions of the binding assay, Ku binding to C3H-NRE1 microcircles was consistently about 4-fold lower than binding to the GR-NRE1 microcircles.	bind
21269	3	7004	6	13	NULL	NULL	NULL	statement 1	Process		is lower than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_9_5647_s_112	9038175	2 However, over several repetitions of the binding assay, Ku binding to C3H-NRE1 microcircles was consistently about 4-fold lower than binding to the GR-NRE1 microcircles.	bind
25384	1	7004	7	10	NULL	0	NULL	Ku	NULL		binds to	NULL					NULL			C3H-NRE1 microcircles	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_9_5647_s_112	9038175	2 However, over several repetitions of the binding assay, Ku binding to C3H-NRE1 microcircles was consistently about 4-fold lower than binding to the GR-NRE1 microcircles.	bind
25385	2	7004	7	10	NULL	0	NULL	Ku	NULL		binds to	NULL					NULL			GR-NRE1 microcircles	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_9_5647_s_112	9038175	2 However, over several repetitions of the binding assay, Ku binding to C3H-NRE1 microcircles was consistently about 4-fold lower than binding to the GR-NRE1 microcircles.	bind
25386	3	7004	7	NULL	NULL	0	NULL	statement 1	NULL		is lower than	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_9_5647_s_112	9038175	2 However, over several repetitions of the binding assay, Ku binding to C3H-NRE1 microcircles was consistently about 4-fold lower than binding to the GR-NRE1 microcircles.	bind
21270	1	7005	6	13	NULL	NULL	NULL	myosin	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_1_668_s_19	16186114	2 However, these myosin-ligand complexes promote an open switch II conformation of myosin (compared with the closed switch II conformation of M-ADP-Pi) (  -  ) and may also change the mechanism of myosin binding to actin.	bind
21271	2	7005	6	13	NULL	NULL	NULL	myosin-ligand complexes	GP		promote					myosin	GP	open switch II conformation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_1_668_s_19	16186114	2 However, these myosin-ligand complexes promote an open switch II conformation of myosin (compared with the closed switch II conformation of M-ADP-Pi) (  -  ) and may also change the mechanism of myosin binding to actin.	bind
21273	4	7005	6	13	NULL	NULL	NULL	myosin-ligand complexes	GP		change		may			statement 1	Process	mechanism of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_1_668_s_19	16186114	2 However, these myosin-ligand complexes promote an open switch II conformation of myosin (compared with the closed switch II conformation of M-ADP-Pi) (  -  ) and may also change the mechanism of myosin binding to actin.	bind
25387	1	7005	7	NULL	NULL	0	NULL	myosin	NULL		bind	NULL				actin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_668_s_19	16186114	2 However, these myosin-ligand complexes promote an open switch II conformation of myosin (compared with the closed switch II conformation of M-ADP-Pi) (  -  ) and may also change the mechanism of myosin binding to actin.	bind
25388	2	7005	7	NULL	NULL	0	NULL	myosin-ligand complexes	NULL		promote	NULL				myosin	NULL	open switch II conformation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_668_s_19	16186114	2 However, these myosin-ligand complexes promote an open switch II conformation of myosin (compared with the closed switch II conformation of M-ADP-Pi) (  -  ) and may also change the mechanism of myosin binding to actin.	bind
25390	3	7005	7	NULL	NULL	0	NULL	myosin-ligand complexes	NULL		change	NULL	may			statement 1	NULL	mechanism of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_668_s_19	16186114	2 However, these myosin-ligand complexes promote an open switch II conformation of myosin (compared with the closed switch II conformation of M-ADP-Pi) (  -  ) and may also change the mechanism of myosin binding to actin.	bind
21274	1	7006	6	13	NULL	NULL	NULL	X11L molecule	GP		bind					APP	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49448_s_272	12972431	2 However, we cannot rule out the possibility that more than one X11L molecule is bound to APP because both X11s could form homo- and/or heterodimers when the respective proteins were overexpressed in cells.	bind
21275	2	7006	6	13	NULL	NULL	NULL	X11L molecule	GP		bind					X11L molecule	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49448_s_272	12972431	2 However, we cannot rule out the possibility that more than one X11L molecule is bound to APP because both X11s could form homo- and/or heterodimers when the respective proteins were overexpressed in cells.	bind
53259	3	7006	6	13	NULL	NULL	NULL	statement 1	Process		forms					heterodimer	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49448_s_272	12972431	2 However, we cannot rule out the possibility that more than one X11L molecule is bound to APP because both X11s could form homo- and/or heterodimers when the respective proteins were overexpressed in cells.	bind
53260	4	7006	6	13	NULL	NULL	NULL	statement 2	Process		forms					homodimer	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49448_s_272	12972431	2 However, we cannot rule out the possibility that more than one X11L molecule is bound to APP because both X11s could form homo- and/or heterodimers when the respective proteins were overexpressed in cells.	bind
25391	1	7006	7	NULL	NULL	0	NULL	X11L molecule	NULL		bind	NULL				APP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49448_s_272	12972431	2 However, we cannot rule out the possibility that more than one X11L molecule is bound to APP because both X11s could form homo- and/or heterodimers when the respective proteins were overexpressed in cells.	bind
25392	2	7006	7	10	NULL	0	NULL	X11 molecule	NULL		bind	NULL				X11 molecule	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49448_s_272	12972431	2 However, we cannot rule out the possibility that more than one X11L molecule is bound to APP because both X11s could form homo- and/or heterodimers when the respective proteins were overexpressed in cells.	bind
25393	3	7006	7	10	NULL	0	NULL	statement 1	NULL		form	NULL				heterodimer	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49448_s_272	12972431	2 However, we cannot rule out the possibility that more than one X11L molecule is bound to APP because both X11s could form homo- and/or heterodimers when the respective proteins were overexpressed in cells.	bind
53258	4	7006	7	10	NULL	0	NULL	statement 2	NULL		forms	NULL				homodimer	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49448_s_272	12972431	2 However, we cannot rule out the possibility that more than one X11L molecule is bound to APP because both X11s could form homo- and/or heterodimers when the respective proteins were overexpressed in cells.	bind
21276	1	7007	6	13	NULL	NULL	NULL	BMP-2	GP		bind					BMPR-II 	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_35_21345_s_40	8702914	2 Human BMPR-II was recently cloned, and it was shown that BMP-2, BMP-4, and OP-1/BMP-7 bound to BMPR-II and transduced signals in combination with certain type I receptors after forming heteromeric complexes ( 35,  36,  37).	bind
21277	2	7007	6	13	NULL	NULL	NULL	BMP-4	GP		bind					BMPR-II	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_35_21345_s_40	8702914	2 Human BMPR-II was recently cloned, and it was shown that BMP-2, BMP-4, and OP-1/BMP-7 bound to BMPR-II and transduced signals in combination with certain type I receptors after forming heteromeric complexes ( 35,  36,  37).	bind
21278	3	7007	6	13	NULL	NULL	NULL	OP-1/BMP-7	GP		bind					BMPR-II	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_35_21345_s_40	8702914	2 Human BMPR-II was recently cloned, and it was shown that BMP-2, BMP-4, and OP-1/BMP-7 bound to BMPR-II and transduced signals in combination with certain type I receptors after forming heteromeric complexes ( 35,  36,  37).	bind
25394	1	7007	7	13	NULL	NULL	NULL	BMP-2	GP		bind					BMPR-II	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_35_21345_s_40	8702914	2 Human BMPR-II was recently cloned, and it was shown that BMP-2, BMP-4, and OP-1/BMP-7 bound to BMPR-II and transduced signals in combination with certain type I receptors after forming heteromeric complexes ( 35,  36,  37).	bind
25395	2	7007	7	13	NULL	NULL	NULL	BMP-4	GP		bind					BMPR-II	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_35_21345_s_40	8702914	2 Human BMPR-II was recently cloned, and it was shown that BMP-2, BMP-4, and OP-1/BMP-7 bound to BMPR-II and transduced signals in combination with certain type I receptors after forming heteromeric complexes ( 35,  36,  37).	bind
25396	3	7007	7	13	NULL	NULL	NULL	OP-1/BMP-7	GP		bind					BMPR-II	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_35_21345_s_40	8702914	2 Human BMPR-II was recently cloned, and it was shown that BMP-2, BMP-4, and OP-1/BMP-7 bound to BMPR-II and transduced signals in combination with certain type I receptors after forming heteromeric complexes ( 35,  36,  37).	bind
25400	8	7007	7	13	NULL	NULL	NULL	statement 5	GP		transduce					signals	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_35_21345_s_40	8702914	2 Human BMPR-II was recently cloned, and it was shown that BMP-2, BMP-4, and OP-1/BMP-7 bound to BMPR-II and transduced signals in combination with certain type I receptors after forming heteromeric complexes ( 35,  36,  37).	bind
25401	9	7007	7	13	NULL	NULL	NULL	statement 6	GP		transduce					signals	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_35_21345_s_40	8702914	2 Human BMPR-II was recently cloned, and it was shown that BMP-2, BMP-4, and OP-1/BMP-7 bound to BMPR-II and transduced signals in combination with certain type I receptors after forming heteromeric complexes ( 35,  36,  37).	bind
25402	7	7007	7	13	NULL	NULL	NULL	statement 4	GP		transduce					signals	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_35_21345_s_40	8702914	2 Human BMPR-II was recently cloned, and it was shown that BMP-2, BMP-4, and OP-1/BMP-7 bound to BMPR-II and transduced signals in combination with certain type I receptors after forming heteromeric complexes ( 35,  36,  37).	bind
53261	4	7007	7	13	NULL	NULL	NULL	statement 1	GP		complex with					type I receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_35_21345_s_40	8702914	2 Human BMPR-II was recently cloned, and it was shown that BMP-2, BMP-4, and OP-1/BMP-7 bound to BMPR-II and transduced signals in combination with certain type I receptors after forming heteromeric complexes ( 35,  36,  37).	bind
53262	5	7007	7	13	NULL	NULL	NULL	statement 2	GP		complex with					type I receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_35_21345_s_40	8702914	2 Human BMPR-II was recently cloned, and it was shown that BMP-2, BMP-4, and OP-1/BMP-7 bound to BMPR-II and transduced signals in combination with certain type I receptors after forming heteromeric complexes ( 35,  36,  37).	bind
53263	6	7007	7	13	NULL	NULL	NULL	statement 3	GP		complex with					type I receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_35_21345_s_40	8702914	2 Human BMPR-II was recently cloned, and it was shown that BMP-2, BMP-4, and OP-1/BMP-7 bound to BMPR-II and transduced signals in combination with certain type I receptors after forming heteromeric complexes ( 35,  36,  37).	bind
21279	1	7008	6	13	NULL	NULL	NULL	HuR	GP		is expressed in					HeLa cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_41_39470_s_39	12882963	2 HuR, which is expressed in HeLa cells ( ), also binds the p38 MAPK-responsive COX-2 and TNF AREs (  -  ).	bind
21280	2	7008	6	13	NULL	NULL	NULL	HuR	GP		bind					COX-2	GP	p38 MAPK-responsive			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_41_39470_s_39	12882963	2 HuR, which is expressed in HeLa cells ( ), also binds the p38 MAPK-responsive COX-2 and TNF AREs (  -  ).	bind
21281	3	7008	6	13	NULL	NULL	NULL	HuR	GP		bind					TNF	NucleicAcid			ARE	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_41_39470_s_39	12882963	2 HuR, which is expressed in HeLa cells ( ), also binds the p38 MAPK-responsive COX-2 and TNF AREs (  -  ).	bind
25403	2	7008	7	10	NULL	0	NULL	HuR	NULL		binds	NULL				COX-2	NULL	p38 MAPK-responsive			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_41_39470_s_39	12882963	2 HuR, which is expressed in HeLa cells ( ), also binds the p38 MAPK-responsive COX-2 and TNF AREs (  -  ).	bind
25404	3	7008	7	10	NULL	0	NULL	HuR	NULL		binds	NULL				TNF	NULL			ARE	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_41_39470_s_39	12882963	2 HuR, which is expressed in HeLa cells ( ), also binds the p38 MAPK-responsive COX-2 and TNF AREs (  -  ).	bind
46414	1	7008	7	10	NULL	0	NULL	HuR	NULL		is expressed in	NULL				HeLa cells	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_41_39470_s_39	12882963	2 HuR, which is expressed in HeLa cells ( ), also binds the p38 MAPK-responsive COX-2 and TNF AREs (  -  ).	bind
21282	1	7009	6	13	NULL	NULL	NULL	Fe2+	Chemical		bind					membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_23_16213_s_310	10347176	2 If a fraction of added Fe2+ is bound to the membranes, ascorbate, etc., the true binding affinity of Fe2+ will be higher than the calculated affinity, but the relative difference in Rb+-  versus Na+-containing media will remain.	bind
21283	2	7009	6	13	NULL	NULL	NULL	Fe2+	Chemical		bind					ascorbate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_23_16213_s_310	10347176	2 If a fraction of added Fe2+ is bound to the membranes, ascorbate, etc., the true binding affinity of Fe2+ will be higher than the calculated affinity, but the relative difference in Rb+-  versus Na+-containing media will remain.	bind
25405	1	7009	7	NULL	NULL	0	NULL	Fe2+	NULL		binds	NULL				membranes	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_23_16213_s_310	10347176	2 If a fraction of added Fe2+ is bound to the membranes, ascorbate, etc., the true binding affinity of Fe2+ will be higher than the calculated affinity, but the relative difference in Rb+-  versus Na+-containing media will remain.	bind
25406	2	7009	7	NULL	NULL	0	NULL	Fe2+	NULL		binds	NULL				ascorbate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_23_16213_s_310	10347176	2 If a fraction of added Fe2+ is bound to the membranes, ascorbate, etc., the true binding affinity of Fe2+ will be higher than the calculated affinity, but the relative difference in Rb+-  versus Na+-containing media will remain.	bind
23094	1	7010	6	13	NULL	NULL	NULL	hnRNP E1	GP		bind					FR mRNA	NucleicAcid			C/U-rich cis-element	NULL	megaloblastic erythroid precursors	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_41510_s_290	11527973	2 If similar mechanisms are operative during erythroid development, (folate deficiency-induced) homocysteine-mediated augmentation of binding of hnRNP E1 to C/U-rich  cis-elements in mRNAs of FR, 15-lipoxygenase, and alpha-globin should result in coordinated up-regulation of FR and alpha-globin but down-regulation of 15-lipoxygenase in megaloblastic erythroid precursors.	bind
23095	2	7010	6	13	NULL	NULL	NULL	hnRNP E1	GP		bind					15-lipoxygenase mRNA	NucleicAcid			C/U-rich cis-element	NULL	megaloblastic erythroid precursors	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_41510_s_290	11527973	2 If similar mechanisms are operative during erythroid development, (folate deficiency-induced) homocysteine-mediated augmentation of binding of hnRNP E1 to C/U-rich  cis-elements in mRNAs of FR, 15-lipoxygenase, and alpha-globin should result in coordinated up-regulation of FR and alpha-globin but down-regulation of 15-lipoxygenase in megaloblastic erythroid precursors.	bind
23096	3	7010	6	13	NULL	NULL	NULL	hnRNP E1	GP		bind					alpha-globin mRNA	NucleicAcid			C/U-rich cis-element	NULL	megaloblastic erythroid precursors	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_41510_s_290	11527973	2 If similar mechanisms are operative during erythroid development, (folate deficiency-induced) homocysteine-mediated augmentation of binding of hnRNP E1 to C/U-rich  cis-elements in mRNAs of FR, 15-lipoxygenase, and alpha-globin should result in coordinated up-regulation of FR and alpha-globin but down-regulation of 15-lipoxygenase in megaloblastic erythroid precursors.	bind
23097	4	7010	6	13	NULL	NULL	NULL	homocysteine	AminoAcid		augments					statement 1	Process				NULL	megaloblastic erythroid precursors	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_41510_s_290	11527973	2 If similar mechanisms are operative during erythroid development, (folate deficiency-induced) homocysteine-mediated augmentation of binding of hnRNP E1 to C/U-rich  cis-elements in mRNAs of FR, 15-lipoxygenase, and alpha-globin should result in coordinated up-regulation of FR and alpha-globin but down-regulation of 15-lipoxygenase in megaloblastic erythroid precursors.	bind
23098	5	7010	6	13	NULL	NULL	NULL	homocysteine	AminoAcid		augments					statement 2	Process				NULL	megaloblastic erythroid precursors	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_41510_s_290	11527973	2 If similar mechanisms are operative during erythroid development, (folate deficiency-induced) homocysteine-mediated augmentation of binding of hnRNP E1 to C/U-rich  cis-elements in mRNAs of FR, 15-lipoxygenase, and alpha-globin should result in coordinated up-regulation of FR and alpha-globin but down-regulation of 15-lipoxygenase in megaloblastic erythroid precursors.	bind
23099	6	7010	6	13	NULL	NULL	NULL	homocysteine	AminoAcid		augments					statement 3	Process				NULL	megaloblastic erythroid precursors	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_41510_s_290	11527973	2 If similar mechanisms are operative during erythroid development, (folate deficiency-induced) homocysteine-mediated augmentation of binding of hnRNP E1 to C/U-rich  cis-elements in mRNAs of FR, 15-lipoxygenase, and alpha-globin should result in coordinated up-regulation of FR and alpha-globin but down-regulation of 15-lipoxygenase in megaloblastic erythroid precursors.	bind
23100	7	7010	6	13	NULL	NULL	NULL	statement 4	Process		upregulates					FR	GP				NULL	megaloblastic erythroid precursors	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_41510_s_290	11527973	2 If similar mechanisms are operative during erythroid development, (folate deficiency-induced) homocysteine-mediated augmentation of binding of hnRNP E1 to C/U-rich  cis-elements in mRNAs of FR, 15-lipoxygenase, and alpha-globin should result in coordinated up-regulation of FR and alpha-globin but down-regulation of 15-lipoxygenase in megaloblastic erythroid precursors.	bind
23101	8	7010	6	13	NULL	NULL	NULL	statement 6	Process		upregulates					alpha-globin 	GP				NULL	megaloblastic erythroid precursors	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_41510_s_290	11527973	2 If similar mechanisms are operative during erythroid development, (folate deficiency-induced) homocysteine-mediated augmentation of binding of hnRNP E1 to C/U-rich  cis-elements in mRNAs of FR, 15-lipoxygenase, and alpha-globin should result in coordinated up-regulation of FR and alpha-globin but down-regulation of 15-lipoxygenase in megaloblastic erythroid precursors.	bind
23102	9	7010	6	13	NULL	NULL	NULL	statement 5	Process		downregulates					15-lipoxygenase 	GP				NULL	megaloblastic erythroid precursors	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_41510_s_290	11527973	2 If similar mechanisms are operative during erythroid development, (folate deficiency-induced) homocysteine-mediated augmentation of binding of hnRNP E1 to C/U-rich  cis-elements in mRNAs of FR, 15-lipoxygenase, and alpha-globin should result in coordinated up-regulation of FR and alpha-globin but down-regulation of 15-lipoxygenase in megaloblastic erythroid precursors.	bind
25407	1	7010	7	10	NULL	0	NULL	hnRNP E1 	NULL		binds	NULL				FR mRNA	NULL			C/U-rich cis-elements	NULL	megaloblastic erythroid precursors	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_41510_s_290	11527973	2 If similar mechanisms are operative during erythroid development, (folate deficiency-induced) homocysteine-mediated augmentation of binding of hnRNP E1 to C/U-rich  cis-elements in mRNAs of FR, 15-lipoxygenase, and alpha-globin should result in coordinated up-regulation of FR and alpha-globin but down-regulation of 15-lipoxygenase in megaloblastic erythroid precursors.	bind
25408	2	7010	7	10	NULL	0	NULL	hnRNP E1 	NULL		bind	NULL				15-lipoxygenase mRNA	NULL			C/U-rich cis-elements	NULL	megaloblastic erythroid precursors	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_41510_s_290	11527973	2 If similar mechanisms are operative during erythroid development, (folate deficiency-induced) homocysteine-mediated augmentation of binding of hnRNP E1 to C/U-rich  cis-elements in mRNAs of FR, 15-lipoxygenase, and alpha-globin should result in coordinated up-regulation of FR and alpha-globin but down-regulation of 15-lipoxygenase in megaloblastic erythroid precursors.	bind
25409	3	7010	7	10	NULL	0	NULL	hnRNP E1 	NULL		binds	NULL				alpha-globin mRNA	NULL			C/U-rich cis-elements	NULL	megaloblastic erythroid precursors	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_41510_s_290	11527973	2 If similar mechanisms are operative during erythroid development, (folate deficiency-induced) homocysteine-mediated augmentation of binding of hnRNP E1 to C/U-rich  cis-elements in mRNAs of FR, 15-lipoxygenase, and alpha-globin should result in coordinated up-regulation of FR and alpha-globin but down-regulation of 15-lipoxygenase in megaloblastic erythroid precursors.	bind
25410	4	7010	7	10	NULL	0	NULL	homocysteine	NULL		augments	NULL				statement 1	NULL				NULL	megaloblastic erythroid precursors	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_41510_s_290	11527973	2 If similar mechanisms are operative during erythroid development, (folate deficiency-induced) homocysteine-mediated augmentation of binding of hnRNP E1 to C/U-rich  cis-elements in mRNAs of FR, 15-lipoxygenase, and alpha-globin should result in coordinated up-regulation of FR and alpha-globin but down-regulation of 15-lipoxygenase in megaloblastic erythroid precursors.	bind
25411	5	7010	7	10	NULL	0	NULL	homocysteine	NULL		augments	NULL				statement 2	NULL				NULL	megaloblastic erythroid precursors	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_41510_s_290	11527973	2 If similar mechanisms are operative during erythroid development, (folate deficiency-induced) homocysteine-mediated augmentation of binding of hnRNP E1 to C/U-rich  cis-elements in mRNAs of FR, 15-lipoxygenase, and alpha-globin should result in coordinated up-regulation of FR and alpha-globin but down-regulation of 15-lipoxygenase in megaloblastic erythroid precursors.	bind
25412	6	7010	7	10	NULL	0	NULL	homocysteine	NULL		augments	NULL				statement 3	NULL				NULL	megaloblastic erythroid precursors	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_41510_s_290	11527973	2 If similar mechanisms are operative during erythroid development, (folate deficiency-induced) homocysteine-mediated augmentation of binding of hnRNP E1 to C/U-rich  cis-elements in mRNAs of FR, 15-lipoxygenase, and alpha-globin should result in coordinated up-regulation of FR and alpha-globin but down-regulation of 15-lipoxygenase in megaloblastic erythroid precursors.	bind
25413	7	7010	7	10	NULL	0	NULL	statement 1	NULL		upregulates	NULL				FR	NULL				NULL	megaloblastic erythroid precursors	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_41510_s_290	11527973	2 If similar mechanisms are operative during erythroid development, (folate deficiency-induced) homocysteine-mediated augmentation of binding of hnRNP E1 to C/U-rich  cis-elements in mRNAs of FR, 15-lipoxygenase, and alpha-globin should result in coordinated up-regulation of FR and alpha-globin but down-regulation of 15-lipoxygenase in megaloblastic erythroid precursors.	bind
25414	8	7010	7	10	NULL	0	NULL	statement 3	NULL		upregulates	NULL				alpha-globin	NULL				NULL	megaloblastic erythroid precursors	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_41510_s_290	11527973	2 If similar mechanisms are operative during erythroid development, (folate deficiency-induced) homocysteine-mediated augmentation of binding of hnRNP E1 to C/U-rich  cis-elements in mRNAs of FR, 15-lipoxygenase, and alpha-globin should result in coordinated up-regulation of FR and alpha-globin but down-regulation of 15-lipoxygenase in megaloblastic erythroid precursors.	bind
25415	9	7010	7	10	NULL	0	NULL	statement 2	NULL		upregulates	NULL				15-lipoxygenase	NULL				NULL	megaloblastic erythroid precursors	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_41510_s_290	11527973	2 If similar mechanisms are operative during erythroid development, (folate deficiency-induced) homocysteine-mediated augmentation of binding of hnRNP E1 to C/U-rich  cis-elements in mRNAs of FR, 15-lipoxygenase, and alpha-globin should result in coordinated up-regulation of FR and alpha-globin but down-regulation of 15-lipoxygenase in megaloblastic erythroid precursors.	bind
21284	1	7011	6	13	NULL	NULL	NULL	SREBP-1c	GP		does not bind		cooperatively			S14	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_37_34419_s_173	11448969	2 If the  in vitro EMSA is a reflection of the binding of these two factors to the S14 promoter  in vivo, then our results indicate that SREBP-1c and NF-Y do not bind cooperatively to the S14 promoter.	bind
21285	2	7011	6	13	NULL	NULL	NULL	NF-Y	GP		does not bind		cooperatively			S14	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_37_34419_s_173	11448969	2 If the  in vitro EMSA is a reflection of the binding of these two factors to the S14 promoter  in vivo, then our results indicate that SREBP-1c and NF-Y do not bind cooperatively to the S14 promoter.	bind
25416	1	7011	7	NULL	NULL	0	NULL	SREBP-1c	NULL		does not bind	NULL	cooperatively			S14	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_37_34419_s_173	11448969	2 If the  in vitro EMSA is a reflection of the binding of these two factors to the S14 promoter  in vivo, then our results indicate that SREBP-1c and NF-Y do not bind cooperatively to the S14 promoter.	bind
25417	2	7011	7	NULL	NULL	0	NULL	NF-Y 	NULL		does not bind	NULL	cooperatively			S14	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_37_34419_s_173	11448969	2 If the  in vitro EMSA is a reflection of the binding of these two factors to the S14 promoter  in vivo, then our results indicate that SREBP-1c and NF-Y do not bind cooperatively to the S14 promoter.	bind
21287	1	7012	6	13	NULL	NULL	NULL	Rap1A	GP		bind								CRR		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_18_11702_s_66	9115221	2 In a striking contrast, Rap1A bound to CRR yielded stronger signal than that to RBD under the same condition, indicating that it has the ability to bind equally to RBD and to CRR (see also Fig.  1 A).	bind
21288	2	7012	6	13	NULL	NULL	NULL	Rap1A	GP		bind								RBD		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_18_11702_s_66	9115221	2 In a striking contrast, Rap1A bound to CRR yielded stronger signal than that to RBD under the same condition, indicating that it has the ability to bind equally to RBD and to CRR (see also Fig.  1 A).	bind
21289	3	7012	6	13	NULL	NULL	NULL	statement 1	Process		has equal affinity as					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_18_11702_s_66	9115221	2 In a striking contrast, Rap1A bound to CRR yielded stronger signal than that to RBD under the same condition, indicating that it has the ability to bind equally to RBD and to CRR (see also Fig.  1 A).	bind
25418	1	7012	7	NULL	NULL	0	NULL	Rap1A 	NULL		bind	NULL					NULL		CRR		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_18_11702_s_66	9115221	2 In a striking contrast, Rap1A bound to CRR yielded stronger signal than that to RBD under the same condition, indicating that it has the ability to bind equally to RBD and to CRR (see also Fig.  1 A).	bind
25419	2	7012	7	NULL	NULL	0	NULL	Rap1A 	NULL		bind	NULL					NULL		RBD		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_18_11702_s_66	9115221	2 In a striking contrast, Rap1A bound to CRR yielded stronger signal than that to RBD under the same condition, indicating that it has the ability to bind equally to RBD and to CRR (see also Fig.  1 A).	bind
25420	3	7012	7	10	NULL	0	NULL	statement 1	NULL		has equal affinity as	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_18_11702_s_66	9115221	2 In a striking contrast, Rap1A bound to CRR yielded stronger signal than that to RBD under the same condition, indicating that it has the ability to bind equally to RBD and to CRR (see also Fig.  1 A).	bind
21290	1	7013	6	13	NULL	NULL	NULL	HP1	GP		bind		specifically	chromo-domain		H3	AminoAcid	methylated	lysine 9		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_25309_s_259	11316813	2 In accordance with this idea, several groups showed most recently that the chromo-domain of HP1 could bind specifically to methylated lysine 9 of H3 ( 36-38).	bind
25422	1	7013	7	NULL	NULL	0	NULL	HP1	NULL		bind	NULL	specifically	 chromo-domain		H3	NULL	methylated	 lysine 9		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_27_25309_s_259	11316813	2 In accordance with this idea, several groups showed most recently that the chromo-domain of HP1 could bind specifically to methylated lysine 9 of H3 ( 36-38).	bind
21291	1	7014	6	13	NULL	NULL	NULL	IRE1	GP		bind					TRAF2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_35867_s_283	11447214	2 In accordance with this, JNK was activated by ER stress through binding of IRE1 to TRAF2 ( 29), an adaptor protein that couples plasma membrane receptors to the activation of JNK.	bind
21292	2	7014	6	13	NULL	NULL	NULL	ER stress	Process		activates					JNK	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_35867_s_283	11447214	2 In accordance with this, JNK was activated by ER stress through binding of IRE1 to TRAF2 ( 29), an adaptor protein that couples plasma membrane receptors to the activation of JNK.	bind
21293	3	7014	6	13	NULL	NULL	NULL	statement 2	Process		occurs through					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_35867_s_283	11447214	2 In accordance with this, JNK was activated by ER stress through binding of IRE1 to TRAF2 ( 29), an adaptor protein that couples plasma membrane receptors to the activation of JNK.	bind
27016	4	7014	6	13	NULL	NULL	NULL	IRE1	GP		is a type of					plasma membrane receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_35867_s_283	11447214	2 In accordance with this, JNK was activated by ER stress through binding of IRE1 to TRAF2 ( 29), an adaptor protein that couples plasma membrane receptors to the activation of JNK.	bind
27017	5	7014	6	13	NULL	NULL	NULL	TRAF2	GP		is a type of					adaptor protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_35867_s_283	11447214	2 In accordance with this, JNK was activated by ER stress through binding of IRE1 to TRAF2 ( 29), an adaptor protein that couples plasma membrane receptors to the activation of JNK.	bind
25423	1	7014	7	NULL	NULL	0	NULL	 IRE1	NULL		bind	NULL				TRAF2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_35867_s_283	11447214	2 In accordance with this, JNK was activated by ER stress through binding of IRE1 to TRAF2 ( 29), an adaptor protein that couples plasma membrane receptors to the activation of JNK.	bind
25424	2	7014	7	NULL	NULL	0	NULL	plasma membrane receptors	NULL		activates	NULL				JNK	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_35867_s_283	11447214	2 In accordance with this, JNK was activated by ER stress through binding of IRE1 to TRAF2 ( 29), an adaptor protein that couples plasma membrane receptors to the activation of JNK.	bind
25425	3	7014	7	NULL	NULL	0	NULL	TRAF2	NULL		couples	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_35867_s_283	11447214	2 In accordance with this, JNK was activated by ER stress through binding of IRE1 to TRAF2 ( 29), an adaptor protein that couples plasma membrane receptors to the activation of JNK.	bind
25426	4	7014	7	NULL	NULL	0	NULL	ER stress	NULL		activates	NULL				JNK	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_38_35867_s_283	11447214	2 In accordance with this, JNK was activated by ER stress through binding of IRE1 to TRAF2 ( 29), an adaptor protein that couples plasma membrane receptors to the activation of JNK.	bind
25427	5	7014	7	NULL	NULL	0	NULL	statement 4	NULL		occurs through	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_38_35867_s_283	11447214	2 In accordance with this, JNK was activated by ER stress through binding of IRE1 to TRAF2 ( 29), an adaptor protein that couples plasma membrane receptors to the activation of JNK.	bind
28017	6	7014	7	NULL	NULL	0	NULL	TRAF2	NULL		is a type of	NULL				adaptor protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_38_35867_s_283	11447214	2 In accordance with this, JNK was activated by ER stress through binding of IRE1 to TRAF2 ( 29), an adaptor protein that couples plasma membrane receptors to the activation of JNK.	bind
46415	7	7014	7	10	NULL	0	NULL	IRE1	NULL		is a type of	NULL				\tplasma membrane receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_38_35867_s_283	11447214	2 In accordance with this, JNK was activated by ER stress through binding of IRE1 to TRAF2 ( 29), an adaptor protein that couples plasma membrane receptors to the activation of JNK.	bind
21294	1	7015	6	13	NULL	NULL	NULL	LCE	GP	mouse	possesses				promoter			potential		SREBP binding sequence (TCATGCCAG)	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_48_45358_s_290	11567032	2 In addition, analysis of the mouse LCE promoter sequence identified in the Celera data base revealed a potential SREBP binding sequence (TCATGCCAG) located 364 base pairs upstream of exon 1 of the gene.	bind
25862	1	7015	7	NULL	NULL	0	NULL	LCE	NULL	mouse	contains	NULL			promoter		NULL	potential		SREBP binding sequence (TCATGCCAG)	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_48_45358_s_290	11567032	2 In addition, analysis of the mouse LCE promoter sequence identified in the Celera data base revealed a potential SREBP binding sequence (TCATGCCAG) located 364 base pairs upstream of exon 1 of the gene.	bind
21295	1	7016	6	13	NULL	NULL	NULL	HeLa nuclear protein extract	GP		contains					GATA-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_36_22076_s_145	8703016	2 In addition, HeLa nuclear protein extract, which contains GATA-2, but not GATA-1 ( 29), did not bind either the normal or patient oligonucleotide, but did bind to Sp1 as a control.	bind
21296	2	7016	6	13	NULL	NULL	NULL	HeLa nuclear protein extract	GP		does not contain					GATA-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_36_22076_s_145	8703016	2 In addition, HeLa nuclear protein extract, which contains GATA-2, but not GATA-1 ( 29), did not bind either the normal or patient oligonucleotide, but did bind to Sp1 as a control.	bind
21299	3	7016	6	13	NULL	NULL	NULL	HeLa nuclear protein extract	GP		bind					Sp1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_36_22076_s_145	8703016	2 In addition, HeLa nuclear protein extract, which contains GATA-2, but not GATA-1 ( 29), did not bind either the normal or patient oligonucleotide, but did bind to Sp1 as a control.	bind
25428	1	7016	7	NULL	NULL	0	NULL	HeLa nuclear protein extract	NULL		contains	NULL				GATA-2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_36_22076_s_145	8703016	2 In addition, HeLa nuclear protein extract, which contains GATA-2, but not GATA-1 ( 29), did not bind either the normal or patient oligonucleotide, but did bind to Sp1 as a control.	bind
25429	2	7016	7	NULL	NULL	0	NULL	HeLa nuclear protein extract	NULL		does not contain	NULL				GATA-1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_36_22076_s_145	8703016	2 In addition, HeLa nuclear protein extract, which contains GATA-2, but not GATA-1 ( 29), did not bind either the normal or patient oligonucleotide, but did bind to Sp1 as a control.	bind
25432	3	7016	7	NULL	NULL	0	NULL	HeLa nuclear protein extract	NULL		binds	NULL				Sp1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_36_22076_s_145	8703016	2 In addition, HeLa nuclear protein extract, which contains GATA-2, but not GATA-1 ( 29), did not bind either the normal or patient oligonucleotide, but did bind to Sp1 as a control.	bind
21300	1	7017	6	13	NULL	NULL	NULL	FGF-1	GP		bind		high affinity			FGFR2 IIIb	GP	soluble			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2444_s_269	11714710	2 In addition, high affinity binding of both FGF-1 and FGF-7 to soluble FGFR2 IIIb is not dependent on heparin, whereas efficient binding to the native receptor requires heparin ( 19,  50).	bind
21301	2	7017	6	13	NULL	NULL	NULL	FGF-7	GP		bind		high affinity			FGFR2 IIIb	GP	soluble			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2444_s_269	11714710	2 In addition, high affinity binding of both FGF-1 and FGF-7 to soluble FGFR2 IIIb is not dependent on heparin, whereas efficient binding to the native receptor requires heparin ( 19,  50).	bind
21302	3	7017	6	13	NULL	NULL	NULL	statement 1	Process		is not dependent on					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2444_s_269	11714710	2 In addition, high affinity binding of both FGF-1 and FGF-7 to soluble FGFR2 IIIb is not dependent on heparin, whereas efficient binding to the native receptor requires heparin ( 19,  50).	bind
21303	4	7017	6	13	NULL	NULL	NULL	statement 2	Process		is not dependent on					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2444_s_269	11714710	2 In addition, high affinity binding of both FGF-1 and FGF-7 to soluble FGFR2 IIIb is not dependent on heparin, whereas efficient binding to the native receptor requires heparin ( 19,  50).	bind
21304	5	7017	6	13	NULL	NULL	NULL	FGF-1	GP		bind		efficiently			receptor	GP	native			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2444_s_269	11714710	2 In addition, high affinity binding of both FGF-1 and FGF-7 to soluble FGFR2 IIIb is not dependent on heparin, whereas efficient binding to the native receptor requires heparin ( 19,  50).	bind
27018	6	7017	6	13	NULL	NULL	NULL	FGF-7	GP		bind		efficiently			receptor	GP	native			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2444_s_269	11714710	2 In addition, high affinity binding of both FGF-1 and FGF-7 to soluble FGFR2 IIIb is not dependent on heparin, whereas efficient binding to the native receptor requires heparin ( 19,  50).	bind
27019	7	7017	6	13	NULL	NULL	NULL	statement 5	Process		requires					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2444_s_269	11714710	2 In addition, high affinity binding of both FGF-1 and FGF-7 to soluble FGFR2 IIIb is not dependent on heparin, whereas efficient binding to the native receptor requires heparin ( 19,  50).	bind
27020	8	7017	6	13	NULL	NULL	NULL	statement 6	Process		requires					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2444_s_269	11714710	2 In addition, high affinity binding of both FGF-1 and FGF-7 to soluble FGFR2 IIIb is not dependent on heparin, whereas efficient binding to the native receptor requires heparin ( 19,  50).	bind
25433	1	7017	7	NULL	NULL	0	NULL	FGF-1	NULL		bind	NULL	high affinity			FGFR2 IIIb 	NULL	soluble			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2444_s_269	11714710	2 In addition, high affinity binding of both FGF-1 and FGF-7 to soluble FGFR2 IIIb is not dependent on heparin, whereas efficient binding to the native receptor requires heparin ( 19,  50).	bind
25434	2	7017	7	NULL	NULL	0	NULL	FGF-7	NULL		bind	NULL	high affinity			FGFR2 IIIb	NULL	soluble			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2444_s_269	11714710	2 In addition, high affinity binding of both FGF-1 and FGF-7 to soluble FGFR2 IIIb is not dependent on heparin, whereas efficient binding to the native receptor requires heparin ( 19,  50).	bind
25435	3	7017	7	NULL	NULL	0	NULL	statement 1	NULL		does not depend on	NULL				heparin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2444_s_269	11714710	2 In addition, high affinity binding of both FGF-1 and FGF-7 to soluble FGFR2 IIIb is not dependent on heparin, whereas efficient binding to the native receptor requires heparin ( 19,  50).	bind
25436	4	7017	7	NULL	NULL	0	NULL	statement 2	NULL		does not depend on	NULL				heparin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2444_s_269	11714710	2 In addition, high affinity binding of both FGF-1 and FGF-7 to soluble FGFR2 IIIb is not dependent on heparin, whereas efficient binding to the native receptor requires heparin ( 19,  50).	bind
25437	5	7017	7	NULL	NULL	0	NULL	FGF-1	NULL		bind	NULL				FGFR2 IIIb	NULL	native receptor			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2444_s_269	11714710	2 In addition, high affinity binding of both FGF-1 and FGF-7 to soluble FGFR2 IIIb is not dependent on heparin, whereas efficient binding to the native receptor requires heparin ( 19,  50).	bind
25438	6	7017	7	NULL	NULL	0	NULL	FGF-7	NULL		bind	NULL				FGFR2 IIIb	NULL	native receptor			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2444_s_269	11714710	2 In addition, high affinity binding of both FGF-1 and FGF-7 to soluble FGFR2 IIIb is not dependent on heparin, whereas efficient binding to the native receptor requires heparin ( 19,  50).	bind
25439	7	7017	7	NULL	NULL	0	NULL	statement 5	NULL		requires	NULL				heparin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2444_s_269	11714710	2 In addition, high affinity binding of both FGF-1 and FGF-7 to soluble FGFR2 IIIb is not dependent on heparin, whereas efficient binding to the native receptor requires heparin ( 19,  50).	bind
25440	8	7017	7	NULL	NULL	0	NULL	statement 6	NULL		requires	NULL				heparin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2444_s_269	11714710	2 In addition, high affinity binding of both FGF-1 and FGF-7 to soluble FGFR2 IIIb is not dependent on heparin, whereas efficient binding to the native receptor requires heparin ( 19,  50).	bind
21306	1	7018	6	13	NULL	NULL	NULL	thrombin	GP		bind					thrombomodulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_45_28168_s_265	8910432	2 In addition, the binding of thrombin to thrombomodulin fixes the active site of the otherwise soluble enzyme at a specific height above the membrane surface ( 12).	bind
25441	1	7018	7	NULL	NULL	0	NULL	thrombin	NULL		bind	NULL				thrombomodulin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_45_28168_s_265	8910432	2 In addition, the binding of thrombin to thrombomodulin fixes the active site of the otherwise soluble enzyme at a specific height above the membrane surface ( 12).	bind
21308	1	7019	6	13	NULL	NULL	NULL	ficolin	GP	recombinant;;wild-type	does not bind					GlcNAc	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_8_6534_s_174	14660572	2 In addition, we are unable to explain why the majority of recombinant wild-type ficolin did not bind the GlcNAc column.	bind
25442	1	7019	7	10	NULL	0	NULL	ficolin	NULL	recombinant;;wild-type	does not bind	NULL				GlcNAc column	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_8_6534_s_174	14660572	2 In addition, we are unable to explain why the majority of recombinant wild-type ficolin did not bind the GlcNAc column.	bind
21309	1	7020	6	13	NULL	NULL	NULL	tsf: su coat proteins	GP		bind					GroEL	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_17_17473_s_350	14764588	2 In agreement with the  in vitro results presented here, our recent  in vivo experiments also show that not only is a higher percentage of  tsf: su coat proteins bound to GroEL than their  tsf parents, but the  tsf: su coat proteins actually induce GroEL expression as compared with the induced GroEL levels for the  tsf coat proteins.	bind
21310	2	7020	6	13	NULL	NULL	NULL	tsf	GP		bind					GroEL	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_17_17473_s_350	14764588	2 In agreement with the  in vitro results presented here, our recent  in vivo experiments also show that not only is a higher percentage of  tsf: su coat proteins bound to GroEL than their  tsf parents, but the  tsf: su coat proteins actually induce GroEL expression as compared with the induced GroEL levels for the  tsf coat proteins.	bind
21311	3	7020	6	13	NULL	NULL	NULL	statement 1	GP	affinity of	is higher than					statement 2	GP	affinity of			NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_17_17473_s_350	14764588	2 In agreement with the  in vitro results presented here, our recent  in vivo experiments also show that not only is a higher percentage of  tsf: su coat proteins bound to GroEL than their  tsf parents, but the  tsf: su coat proteins actually induce GroEL expression as compared with the induced GroEL levels for the  tsf coat proteins.	bind
21312	4	7020	6	13	NULL	NULL	NULL	tsf: su coat proteins	GP		induce					GroEL	GP	expression of			NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_17_17473_s_350	14764588	2 In agreement with the  in vitro results presented here, our recent  in vivo experiments also show that not only is a higher percentage of  tsf: su coat proteins bound to GroEL than their  tsf parents, but the  tsf: su coat proteins actually induce GroEL expression as compared with the induced GroEL levels for the  tsf coat proteins.	bind
25443	1	7020	7	NULL	NULL	0	NULL	tsf: su coat proteins	NULL		bind	NULL				GroEL	NULL				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_17_17473_s_350	14764588	2 In agreement with the  in vitro results presented here, our recent  in vivo experiments also show that not only is a higher percentage of  tsf: su coat proteins bound to GroEL than their  tsf parents, but the  tsf: su coat proteins actually induce GroEL expression as compared with the induced GroEL levels for the  tsf coat proteins.	bind
25444	2	7020	7	NULL	NULL	0	NULL	tsf	NULL		bind	NULL				GroEL	NULL				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_17_17473_s_350	14764588	2 In agreement with the  in vitro results presented here, our recent  in vivo experiments also show that not only is a higher percentage of  tsf: su coat proteins bound to GroEL than their  tsf parents, but the  tsf: su coat proteins actually induce GroEL expression as compared with the induced GroEL levels for the  tsf coat proteins.	bind
25445	3	7020	7	10	NULL	0	NULL	statement 1	NULL	affinity of	is greater than	NULL				statement 2	NULL	affinity of			NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_17_17473_s_350	14764588	2 In agreement with the  in vitro results presented here, our recent  in vivo experiments also show that not only is a higher percentage of  tsf: su coat proteins bound to GroEL than their  tsf parents, but the  tsf: su coat proteins actually induce GroEL expression as compared with the induced GroEL levels for the  tsf coat proteins.	bind
25446	4	7020	7	10	NULL	0	NULL	 tsf: su coat proteins 	NULL		induce	NULL				GroEL	NULL	expression of			NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_17_17473_s_350	14764588	2 In agreement with the  in vitro results presented here, our recent  in vivo experiments also show that not only is a higher percentage of  tsf: su coat proteins bound to GroEL than their  tsf parents, but the  tsf: su coat proteins actually induce GroEL expression as compared with the induced GroEL levels for the  tsf coat proteins.	bind
21313	1	7021	6	13	NULL	NULL	NULL	integrin	GP		adopts			I-domain				classic	dinucleotide binding fold		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25162_s_25	9312128	2 In all cases, the integrin I-domain adopts the classic "`dinucleotide binding"` fold with a central hydrophobic parallel beta-sheet, flanked on two sides by amphipathic helices ( 10).	bind
21314	2	7021	6	13	NULL	NULL	NULL	integrin	GP	classic	contains			dinucleotide binding fold				central hydrophobic parallel	beta sheet		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25162_s_25	9312128	2 In all cases, the integrin I-domain adopts the classic "`dinucleotide binding"` fold with a central hydrophobic parallel beta-sheet, flanked on two sides by amphipathic helices ( 10).	bind
21315	3	7021	6	13	NULL	NULL	NULL	integrin	GP	classic	is flanked by			dinucleotide binding fold					amphipathic helices		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25162_s_25	9312128	2 In all cases, the integrin I-domain adopts the classic "`dinucleotide binding"` fold with a central hydrophobic parallel beta-sheet, flanked on two sides by amphipathic helices ( 10).	bind
25447	1	7021	7	NULL	NULL	0	NULL	integrin	NULL		adopts	NULL		 I-domain			NULL	classic	dinucleotide binding fold		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25162_s_25	9312128	2 In all cases, the integrin I-domain adopts the classic "`dinucleotide binding"` fold with a central hydrophobic parallel beta-sheet, flanked on two sides by amphipathic helices ( 10).	bind
25448	2	7021	7	10	NULL	0	NULL	integrin	NULL	classic	contain	NULL		dinucleotide binding fold			NULL	 central hydrophobic parallel	beta-sheet		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25162_s_25	9312128	2 In all cases, the integrin I-domain adopts the classic "`dinucleotide binding"` fold with a central hydrophobic parallel beta-sheet, flanked on two sides by amphipathic helices ( 10).	bind
25449	3	7021	7	10	NULL	0	NULL	integrin	NULL	classic	flanked by	NULL		dinucleotide binding fold			NULL		amphipathic helices		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25162_s_25	9312128	2 In all cases, the integrin I-domain adopts the classic "`dinucleotide binding"` fold with a central hydrophobic parallel beta-sheet, flanked on two sides by amphipathic helices ( 10).	bind
21316	1	7022	6	13	NULL	NULL	NULL	PTPD1	GP		bind								PH domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_52_41124_s_278	11013262	2 In consideration of the molecular mechanism regulating Etk activity, it is likely that the binding of PTPD1 to the PH domain dissociates the intramolecular interaction between the PH domain and other subdomains of Etk, leading to Etk in an open conformation and kinase-active state.	bind
21317	2	7022	6	13	NULL	NULL	NULL	Etk	GP		interacts with		intramolecularly	PH domain		Etk	GP		subdomains		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_52_41124_s_278	11013262	2 In consideration of the molecular mechanism regulating Etk activity, it is likely that the binding of PTPD1 to the PH domain dissociates the intramolecular interaction between the PH domain and other subdomains of Etk, leading to Etk in an open conformation and kinase-active state.	bind
21318	3	7022	6	13	NULL	NULL	NULL	statement 1	Process		dissociates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_52_41124_s_278	11013262	2 In consideration of the molecular mechanism regulating Etk activity, it is likely that the binding of PTPD1 to the PH domain dissociates the intramolecular interaction between the PH domain and other subdomains of Etk, leading to Etk in an open conformation and kinase-active state.	bind
21319	4	7022	6	13	NULL	NULL	NULL	statement 3	Process		leads to					Etk	GP	open conformation of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_52_41124_s_278	11013262	2 In consideration of the molecular mechanism regulating Etk activity, it is likely that the binding of PTPD1 to the PH domain dissociates the intramolecular interaction between the PH domain and other subdomains of Etk, leading to Etk in an open conformation and kinase-active state.	bind
25450	1	7022	7	NULL	NULL	0	NULL	PTPD1	NULL		bind	NULL				Etk	NULL		PH domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_52_41124_s_278	11013262	2 In consideration of the molecular mechanism regulating Etk activity, it is likely that the binding of PTPD1 to the PH domain dissociates the intramolecular interaction between the PH domain and other subdomains of Etk, leading to Etk in an open conformation and kinase-active state.	bind
25451	2	7022	7	10	NULL	0	NULL	Etk	NULL		interacts with	NULL	intramolecular	PH domain		Etk	NULL		subdomains		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_52_41124_s_278	11013262	2 In consideration of the molecular mechanism regulating Etk activity, it is likely that the binding of PTPD1 to the PH domain dissociates the intramolecular interaction between the PH domain and other subdomains of Etk, leading to Etk in an open conformation and kinase-active state.	bind
25452	3	7022	7	NULL	NULL	0	NULL	statement 1	NULL		dissociates	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_52_41124_s_278	11013262	2 In consideration of the molecular mechanism regulating Etk activity, it is likely that the binding of PTPD1 to the PH domain dissociates the intramolecular interaction between the PH domain and other subdomains of Etk, leading to Etk in an open conformation and kinase-active state.	bind
25453	4	7022	7	NULL	NULL	0	NULL	statement 3	NULL		leads to	NULL				Etk	NULL	open conformation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_52_41124_s_278	11013262	2 In consideration of the molecular mechanism regulating Etk activity, it is likely that the binding of PTPD1 to the PH domain dissociates the intramolecular interaction between the PH domain and other subdomains of Etk, leading to Etk in an open conformation and kinase-active state.	bind
25454	5	7022	7	NULL	NULL	0	NULL	statement 3	NULL		leads to	NULL				Etk	NULL	kinase-active state of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_52_41124_s_278	11013262	2 In consideration of the molecular mechanism regulating Etk activity, it is likely that the binding of PTPD1 to the PH domain dissociates the intramolecular interaction between the PH domain and other subdomains of Etk, leading to Etk in an open conformation and kinase-active state.	bind
21320	1	7023	6	13	NULL	NULL	NULL	TARC receptor	GP	T cell	specific for		highly			TARC	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_35_21514_s_240	8702936	2 In contrast to other known CC chemokine receptors that usually bind more than one chemokine, the TARC receptor on T cells appears to be highly specific for TARC.	bind
21321	2	7023	6	13	NULL	NULL	NULL	CC chemokine receptors	GP		bind					chemokine	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_35_21514_s_240	8702936	2 In contrast to other known CC chemokine receptors that usually bind more than one chemokine, the TARC receptor on T cells appears to be highly specific for TARC.	bind
25455	1	7023	7	NULL	NULL	0	NULL	CC chemokine receptors	NULL		bind	NULL				chemokine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_35_21514_s_240	8702936	2 In contrast to other known CC chemokine receptors that usually bind more than one chemokine, the TARC receptor on T cells appears to be highly specific for TARC.	bind
25456	2	7023	7	10	NULL	0	NULL	TARC receptor	NULL	T cells	specific for	NULL	highly			TARC	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_35_21514_s_240	8702936	2 In contrast to other known CC chemokine receptors that usually bind more than one chemokine, the TARC receptor on T cells appears to be highly specific for TARC.	bind
21322	1	7024	6	13	NULL	NULL	NULL	paxillin fragment	GP	expression of	failed to bind								alpha 4 tail		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_23_20887_s_208	11919182	2 In contrast, expression of a fragment of paxillin that failed to bind to the alpha4 tail, P(Met1-Lys125), did not inhibit cell migration on fibrinogen (Fig.  7 A, left panel).	bind
21323	2	7024	6	13	NULL	NULL	NULL	fibrinogen	GP		did not inhibit			P(Met1-Lys125)		cell migration	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_23_20887_s_208	11919182	2 In contrast, expression of a fragment of paxillin that failed to bind to the alpha4 tail, P(Met1-Lys125), did not inhibit cell migration on fibrinogen (Fig.  7 A, left panel).	bind
25457	1	7024	7	NULL	NULL	0	NULL	 paxillin fragment	NULL		does not bind	NULL					NULL		  alpha4 tail		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_23_20887_s_208	11919182	2 In contrast, expression of a fragment of paxillin that failed to bind to the alpha4 tail, P(Met1-Lys125), did not inhibit cell migration on fibrinogen (Fig.  7 A, left panel).	bind
25458	2	7024	7	NULL	NULL	0	NULL	paxillin fragment	NULL		does not bind	NULL					NULL		P(Met1-Lys125)		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_23_20887_s_208	11919182	2 In contrast, expression of a fragment of paxillin that failed to bind to the alpha4 tail, P(Met1-Lys125), did not inhibit cell migration on fibrinogen (Fig.  7 A, left panel).	bind
25459	3	7024	7	NULL	NULL	0	NULL	paxillin fragment	NULL		does not inhibit	NULL				fibrinogen	NULL	cell migration on			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_23_20887_s_208	11919182	2 In contrast, expression of a fragment of paxillin that failed to bind to the alpha4 tail, P(Met1-Lys125), did not inhibit cell migration on fibrinogen (Fig.  7 A, left panel).	bind
21324	1	7025	6	13	NULL	NULL	NULL	CD151	GP		associates with					CD9	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
21325	2	7025	6	13	NULL	NULL	NULL	CD151	GP		associates with					CD81	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
21326	3	7025	6	13	NULL	NULL	NULL	alpha3beta1	GP		associates with					CD9	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
21327	4	7025	6	13	NULL	NULL	NULL	alpha3beta1	GP		associates with					CD81	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
21328	5	7025	6	13	NULL	NULL	NULL	alpha6beta1	GP		associates with					CD9	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
21329	6	7025	6	13	NULL	NULL	NULL	alpha6beta1	GP		associates with					CD81	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
21330	7	7025	6	13	NULL	NULL	NULL	EWI-2	GP		does not associate with					alpha 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
21331	8	7025	6	13	NULL	NULL	NULL	EWI-2	GP		does not associate with					alpha3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
21332	9	7025	6	13	NULL	NULL	NULL	EWI-2	GP		does not associate with					alpha6	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
21333	10	7025	6	13	NULL	NULL	NULL	EWI-2	GP		does not associate with					beta1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
21334	11	7025	6	13	NULL	NULL	NULL	EWI-2	GP		does not associate with					CD151	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
21335	12	7025	6	13	NULL	NULL	NULL	EWI-F	GP		does not associate with					alpha2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
21336	13	7025	6	13	NULL	NULL	NULL	EWI-F	GP		does not associate with					alpha3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
21337	14	7025	6	13	NULL	NULL	NULL	EWI-F	GP		does not associate with					alpha6	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
21338	15	7025	6	13	NULL	NULL	NULL	EWI-F	GP		does not associate with					beta1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
21339	16	7025	6	13	NULL	NULL	NULL	EWI-F	GP		does not associate with					CD151	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
25460	1	7025	7	NULL	NULL	0	NULL	CD151	NULL		associate with	NULL				CD9	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
25461	2	7025	7	NULL	NULL	0	NULL	alpha3beta1	NULL		associate with	NULL				CD9	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
25462	3	7025	7	NULL	NULL	0	NULL	alpha6beta1 	NULL		associate with	NULL				CD9	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
25463	4	7025	7	NULL	NULL	0	NULL	CD151	NULL		associate with	NULL				CD81	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
25464	5	7025	7	NULL	NULL	0	NULL	alpha3beta1	NULL		associate with	NULL				CD81	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
25465	6	7025	7	NULL	NULL	0	NULL	alpha6beta1	NULL		associate with	NULL				CD81	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
25466	7	7025	7	NULL	NULL	0	NULL	EWI-2	NULL		does not associate with	NULL				alpha2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
25467	8	7025	7	NULL	NULL	0	NULL	EWI-2	NULL		does not associate with	NULL				alpha3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
25468	9	7025	7	NULL	NULL	0	NULL	EWI-2	NULL		does not associate with	NULL				alpha6	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
25469	10	7025	7	NULL	NULL	0	NULL	EWI-2	NULL		does not associate with	NULL				beta1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
25470	11	7025	7	NULL	NULL	0	NULL	EWI-2	NULL		does not associate with	NULL				CD151	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
25471	12	7025	7	NULL	NULL	0	NULL	EWI-F	NULL		does not associate with	NULL				alpha2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
25472	13	7025	7	NULL	NULL	0	NULL	EWI-F	NULL		does not associate with	NULL				alpha3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
25473	14	7025	7	NULL	NULL	0	NULL	EWI-F	NULL		does not associate with	NULL				alpha6	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
25474	15	7025	7	NULL	NULL	0	NULL	EWI-F	NULL		does not associate with	NULL				beta1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
25475	16	7025	7	NULL	NULL	0	NULL	EWI-F	NULL		does not associate with	NULL				CD151	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_44_40545_s_296	11504738	2 In contrast, the 293 cellular environment seems to lack an extensive "`tetraspan web"` such that CD151, alpha3beta1, and alpha6beta1 associated with CD9 and CD81 only at a very low stoichiometry ( 30)), and no EWI-2 or EWI-F association with alpha2, alpha3, alpha6, beta1, or CD151 could be detected (Ref.  30 and Fig.  4).	bind
21340	1	7026	6	13	NULL	NULL	NULL	apoA-I	GP		does not bind		significantly			ECM	CellComponent				NULL	efflux-impaired U937 macrophages	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_35_31318_s_297	12050168	2 In contrast, we have been unable to demonstrate significant binding of apoA-I to the ECM of efflux-impaired U937 macrophages or fibroblasts (Fig.  1).	bind
21341	2	7026	6	13	NULL	NULL	NULL	Apo A-I	GP		does not bind		significantly			ECM	CellComponent				NULL	efflux-impaired U937 fibroblasts	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_35_31318_s_297	12050168	2 In contrast, we have been unable to demonstrate significant binding of apoA-I to the ECM of efflux-impaired U937 macrophages or fibroblasts (Fig.  1).	bind
25596	1	7026	7	NULL	NULL	0	NULL	apoA-I 	NULL		does not bind	NULL	significantly			 ECM 	NULL				NULL	efflux-impaired U937 macrophages	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_35_31318_s_297	12050168	2 In contrast, we have been unable to demonstrate significant binding of apoA-I to the ECM of efflux-impaired U937 macrophages or fibroblasts (Fig.  1).	bind
25597	2	7026	7	NULL	NULL	0	NULL	apoA-I	NULL		does not bind	NULL	significantly			ECM	NULL				NULL	efflux-impaired U937 fibroblasts	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_35_31318_s_297	12050168	2 In contrast, we have been unable to demonstrate significant binding of apoA-I to the ECM of efflux-impaired U937 macrophages or fibroblasts (Fig.  1).	bind
22168	1	7027	6	13	NULL	NULL	NULL	glypican	GP		bind					Abeta	GP	fibrillar 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31617_s_216	9395501	2 In future, we plan to use ACE both to refine the characterization of the heparin-binding conformation of Abeta as well as to more thoroughly characterize the binding of intact HSPGs such as glypican and perlecan to fibrillar and nonfibrillar Abeta.	bind
22169	2	7027	6	13	NULL	NULL	NULL	perlecan	GP		bind					Abeta	GP	nonfibrillar			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31617_s_216	9395501	2 In future, we plan to use ACE both to refine the characterization of the heparin-binding conformation of Abeta as well as to more thoroughly characterize the binding of intact HSPGs such as glypican and perlecan to fibrillar and nonfibrillar Abeta.	bind
22170	3	7027	6	13	NULL	NULL	NULL	Abeta	GP		bind					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31617_s_216	9395501	2 In future, we plan to use ACE both to refine the characterization of the heparin-binding conformation of Abeta as well as to more thoroughly characterize the binding of intact HSPGs such as glypican and perlecan to fibrillar and nonfibrillar Abeta.	bind
27021	4	7027	6	13	NULL	NULL	NULL	glypican	GP		is a type of					HSPG	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31617_s_216	9395501	2 In future, we plan to use ACE both to refine the characterization of the heparin-binding conformation of Abeta as well as to more thoroughly characterize the binding of intact HSPGs such as glypican and perlecan to fibrillar and nonfibrillar Abeta.	bind
27022	5	7027	6	13	NULL	NULL	NULL	perlecan	GP		is a type of					HSPG	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31617_s_216	9395501	2 In future, we plan to use ACE both to refine the characterization of the heparin-binding conformation of Abeta as well as to more thoroughly characterize the binding of intact HSPGs such as glypican and perlecan to fibrillar and nonfibrillar Abeta.	bind
53264	6	7027	6	13	NULL	NULL	NULL	glypican	GP		bind					Abeta	GP	nonfibrillar			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31617_s_216	9395501	2 In future, we plan to use ACE both to refine the characterization of the heparin-binding conformation of Abeta as well as to more thoroughly characterize the binding of intact HSPGs such as glypican and perlecan to fibrillar and nonfibrillar Abeta.	bind
53265	7	7027	6	13	NULL	NULL	NULL	perlecan	GP		bind					Abeta	GP	fibrillar			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31617_s_216	9395501	2 In future, we plan to use ACE both to refine the characterization of the heparin-binding conformation of Abeta as well as to more thoroughly characterize the binding of intact HSPGs such as glypican and perlecan to fibrillar and nonfibrillar Abeta.	bind
25598	1	7027	7	10	NULL	0	NULL	glypican	NULL		bind	NULL				Abeta	NULL	fibrillar			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31617_s_216	9395501	2 In future, we plan to use ACE both to refine the characterization of the heparin-binding conformation of Abeta as well as to more thoroughly characterize the binding of intact HSPGs such as glypican and perlecan to fibrillar and nonfibrillar Abeta.	bind
25599	2	7027	7	10	NULL	0	NULL	 perlecan	NULL		bind	NULL				Abeta	NULL	fibrillar			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31617_s_216	9395501	2 In future, we plan to use ACE both to refine the characterization of the heparin-binding conformation of Abeta as well as to more thoroughly characterize the binding of intact HSPGs such as glypican and perlecan to fibrillar and nonfibrillar Abeta.	bind
25600	3	7027	7	10	NULL	0	NULL	glypican	NULL		bind	NULL				Abeta	NULL	nonfibrillar			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31617_s_216	9395501	2 In future, we plan to use ACE both to refine the characterization of the heparin-binding conformation of Abeta as well as to more thoroughly characterize the binding of intact HSPGs such as glypican and perlecan to fibrillar and nonfibrillar Abeta.	bind
25601	4	7027	7	10	NULL	0	NULL	Perlecan	NULL		bind	NULL				Abeta	NULL	nonfibrillar			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31617_s_216	9395501	2 In future, we plan to use ACE both to refine the characterization of the heparin-binding conformation of Abeta as well as to more thoroughly characterize the binding of intact HSPGs such as glypican and perlecan to fibrillar and nonfibrillar Abeta.	bind
25602	5	7027	7	NULL	NULL	0	NULL	glypican	NULL		is a type of	NULL				HSPG	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_50_31617_s_216	9395501	2 In future, we plan to use ACE both to refine the characterization of the heparin-binding conformation of Abeta as well as to more thoroughly characterize the binding of intact HSPGs such as glypican and perlecan to fibrillar and nonfibrillar Abeta.	bind
25603	6	7027	7	NULL	NULL	0	NULL	Perlecan	NULL		is a type of	NULL				HSPG	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_50_31617_s_216	9395501	2 In future, we plan to use ACE both to refine the characterization of the heparin-binding conformation of Abeta as well as to more thoroughly characterize the binding of intact HSPGs such as glypican and perlecan to fibrillar and nonfibrillar Abeta.	bind
53266	7	7027	7	10	NULL	0	NULL	Abeta	NULL		bind	NULL				heparin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_50_31617_s_216	9395501	2 In future, we plan to use ACE both to refine the characterization of the heparin-binding conformation of Abeta as well as to more thoroughly characterize the binding of intact HSPGs such as glypican and perlecan to fibrillar and nonfibrillar Abeta.	bind
21342	1	7028	6	13	NULL	NULL	NULL	Cdc42p	AminoAcid		is mutated to			Tyr-40		Cdc42p	AminoAcid		Cys		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7176_s_155	11113154	2 In particular, mutation of Tyr-40 to Cys created a version of Cdc42p largely unable to bind the Cdc42/Rac-interactive binding motif ( 42) common to several effectors ( 43).	bind
21343	2	7028	6	13	NULL	NULL	NULL	Cdc42p	AminoAcid		does not bind			Cys					Cdc42/Rac-interactive binding motif		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7176_s_155	11113154	2 In particular, mutation of Tyr-40 to Cys created a version of Cdc42p largely unable to bind the Cdc42/Rac-interactive binding motif ( 42) common to several effectors ( 43).	bind
25604	1	7028	7	NULL	NULL	0	NULL	Cdc42p	NULL		mutated to	NULL		Tyr-40		Cdc42p	NULL		Cys		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_10_7176_s_155	11113154	2 In particular, mutation of Tyr-40 to Cys created a version of Cdc42p largely unable to bind the Cdc42/Rac-interactive binding motif ( 42) common to several effectors ( 43).	bind
25605	2	7028	7	NULL	NULL	0	NULL	Cdc42p	NULL		does not bind	NULL		Cys			NULL		Cdc42/Rac-interactive binding motif		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_10_7176_s_155	11113154	2 In particular, mutation of Tyr-40 to Cys created a version of Cdc42p largely unable to bind the Cdc42/Rac-interactive binding motif ( 42) common to several effectors ( 43).	bind
21344	1	7029	6	13	NULL	NULL	NULL	MEK	GP	nematode	bind					TAO1	GP	mammalian			NULL		NULL	NULL	NULL	NULL	gw60_gene_279_2_137_s_218	11733138	2 in TAO1-HA immune complexes as well as the converse, indicating that the nematode MEK binds to mammalian TAO1 when the two proteins are co-expressed (  Fig. 8B).	bind
25607	2	7029	7	NULL	NULL	0	NULL	MEK	NULL	nematode	binds	NULL				 TAO1	NULL	mammalian			NULL		NULL	NULL	NULL	NULL	gw60_gene_279_2_137_s_218	11733138	2 in TAO1-HA immune complexes as well as the converse, indicating that the nematode MEK binds to mammalian TAO1 when the two proteins are co-expressed (  Fig. 8B).	bind
21345	1	7030	6	13	NULL	NULL	NULL	cADP	Chemical		bind					ribose	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17739_s_155	8663443	2 In the latter cells, positive results ( 16,  39) have been questioned because of a possible competition of cADP-ribose binding by ATP ( 13,  17,  18).	bind
21346	2	7030	6	13	NULL	NULL	NULL	ATP	Chemical		bind					ribose	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17739_s_155	8663443	2 In the latter cells, positive results ( 16,  39) have been questioned because of a possible competition of cADP-ribose binding by ATP ( 13,  17,  18).	bind
21347	3	7030	6	13	NULL	NULL	NULL	statement 1	Process		competes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17739_s_155	8663443	2 In the latter cells, positive results ( 16,  39) have been questioned because of a possible competition of cADP-ribose binding by ATP ( 13,  17,  18).	bind
25608	1	7030	7	NULL	NULL	0	NULL	cADP	NULL		bind	NULL				ribose	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17739_s_155	8663443	2 In the latter cells, positive results ( 16,  39) have been questioned because of a possible competition of cADP-ribose binding by ATP ( 13,  17,  18).	bind
28022	2	7030	7	NULL	NULL	0	NULL	ATP	NULL		bind	NULL				ribose	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_30_17739_s_155	8663443	2 In the latter cells, positive results ( 16,  39) have been questioned because of a possible competition of cADP-ribose binding by ATP ( 13,  17,  18).	bind
28023	3	7030	7	NULL	NULL	0	NULL	statement 1	NULL		competes	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_30_17739_s_155	8663443	2 In the latter cells, positive results ( 16,  39) have been questioned because of a possible competition of cADP-ribose binding by ATP ( 13,  17,  18).	bind
21348	1	7032	6	13	NULL	NULL	NULL	GST-FinO protein	GP	purified	bind					FinP RNA	NucleicAcid	radiolabeled			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_15_10356_s_69	10187824	2 In the present study, the relative equilibrium association constants for GST-FinO binding to FinP variants were determined by performing gel-shift assays in which radiolabeled RNA was combined with increasing amounts of purified GST-FinO protein.	bind
25611	1	7032	7	10	NULL	0	NULL	GST-FinO protein	NULL	Purified	bind	NULL				FinP RNA	NULL	radiolabeled			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_15_10356_s_69	10187824	2 In the present study, the relative equilibrium association constants for GST-FinO binding to FinP variants were determined by performing gel-shift assays in which radiolabeled RNA was combined with increasing amounts of purified GST-FinO protein.	bind
21349	1	7033	6	13	NULL	NULL	NULL	MEKK1	GP		bind					Axin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_38_39366_s_266	15262978	2 In the present study, we found that like glycogen synthase kinase-3beta and casein kinase Ialpha/epsilon, Ccd1 binding competes against MEKK1 binding to Axin.	bind
21350	2	7033	6	13	NULL	NULL	NULL	Ccd1	GP		bind					Axin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_38_39366_s_266	15262978	2 In the present study, we found that like glycogen synthase kinase-3beta and casein kinase Ialpha/epsilon, Ccd1 binding competes against MEKK1 binding to Axin.	bind
21351	3	7033	6	13	NULL	NULL	NULL	statement 2	Process		competes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_38_39366_s_266	15262978	2 In the present study, we found that like glycogen synthase kinase-3beta and casein kinase Ialpha/epsilon, Ccd1 binding competes against MEKK1 binding to Axin.	bind
21352	4	7033	6	13	NULL	NULL	NULL	glycogen synthase kinase-3beta	GP		bind					Axin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_38_39366_s_266	15262978	2 In the present study, we found that like glycogen synthase kinase-3beta and casein kinase Ialpha/epsilon, Ccd1 binding competes against MEKK1 binding to Axin.	bind
21353	5	7033	6	13	NULL	NULL	NULL	statement 4	Process		competes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_38_39366_s_266	15262978	2 In the present study, we found that like glycogen synthase kinase-3beta and casein kinase Ialpha/epsilon, Ccd1 binding competes against MEKK1 binding to Axin.	bind
21354	6	7033	6	13	NULL	NULL	NULL	casein kinase Ialpha/epsilon	GP		bind					Axin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_38_39366_s_266	15262978	2 In the present study, we found that like glycogen synthase kinase-3beta and casein kinase Ialpha/epsilon, Ccd1 binding competes against MEKK1 binding to Axin.	bind
21355	7	7033	6	13	NULL	NULL	NULL	statement 6	Process		competes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_38_39366_s_266	15262978	2 In the present study, we found that like glycogen synthase kinase-3beta and casein kinase Ialpha/epsilon, Ccd1 binding competes against MEKK1 binding to Axin.	bind
25612	1	7033	7	NULL	NULL	0	NULL	MEKK1	NULL		bind	NULL				Axin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_38_39366_s_266	15262978	2 In the present study, we found that like glycogen synthase kinase-3beta and casein kinase Ialpha/epsilon, Ccd1 binding competes against MEKK1 binding to Axin.	bind
25613	2	7033	7	NULL	NULL	0	NULL	Ccd1	NULL		bind	NULL				Axin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_38_39366_s_266	15262978	2 In the present study, we found that like glycogen synthase kinase-3beta and casein kinase Ialpha/epsilon, Ccd1 binding competes against MEKK1 binding to Axin.	bind
25614	3	7033	7	NULL	NULL	0	NULL	statement 2	NULL		compete with	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_38_39366_s_266	15262978	2 In the present study, we found that like glycogen synthase kinase-3beta and casein kinase Ialpha/epsilon, Ccd1 binding competes against MEKK1 binding to Axin.	bind
25615	4	7033	7	NULL	NULL	0	NULL	glycogen synthase kinase-3beta	NULL		bind	NULL				Axin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_38_39366_s_266	15262978	2 In the present study, we found that like glycogen synthase kinase-3beta and casein kinase Ialpha/epsilon, Ccd1 binding competes against MEKK1 binding to Axin.	bind
25616	5	7033	7	NULL	NULL	0	NULL	casein kinase Ialpha/epsilon	NULL		bind	NULL				Axin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_38_39366_s_266	15262978	2 In the present study, we found that like glycogen synthase kinase-3beta and casein kinase Ialpha/epsilon, Ccd1 binding competes against MEKK1 binding to Axin.	bind
25617	6	7033	7	NULL	NULL	0	NULL	statement 4	NULL		compete with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_38_39366_s_266	15262978	2 In the present study, we found that like glycogen synthase kinase-3beta and casein kinase Ialpha/epsilon, Ccd1 binding competes against MEKK1 binding to Axin.	bind
25618	7	7033	7	NULL	NULL	0	NULL	statement 5	NULL		compete with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_38_39366_s_266	15262978	2 In the present study, we found that like glycogen synthase kinase-3beta and casein kinase Ialpha/epsilon, Ccd1 binding competes against MEKK1 binding to Axin.	bind
21356	1	7034	6	13	NULL	NULL	NULL	p65	GP		is translocated to					nucleus	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_21_2707_s_19	12438297	2 In the stable trimeric complex of p65, p105/50, and IkappaB, IkappaB prevents nuclear translocation and DNA binding of p65 by masking its nuclear localization signal.	bind
21357	2	7034	6	13	NULL	NULL	NULL	p65	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_21_2707_s_19	12438297	2 In the stable trimeric complex of p65, p105/50, and IkappaB, IkappaB prevents nuclear translocation and DNA binding of p65 by masking its nuclear localization signal.	bind
21358	3	7034	6	13	NULL	NULL	NULL	IkappaB	GP		prevents					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_21_2707_s_19	12438297	2 In the stable trimeric complex of p65, p105/50, and IkappaB, IkappaB prevents nuclear translocation and DNA binding of p65 by masking its nuclear localization signal.	bind
21359	4	7034	6	13	NULL	NULL	NULL	IkappaB	GP		prevents					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_21_2707_s_19	12438297	2 In the stable trimeric complex of p65, p105/50, and IkappaB, IkappaB prevents nuclear translocation and DNA binding of p65 by masking its nuclear localization signal.	bind
21360	5	7034	6	13	NULL	NULL	NULL	IkappaB	GP		mask					p65	GP		 nuclear localization signal		NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_21_2707_s_19	12438297	2 In the stable trimeric complex of p65, p105/50, and IkappaB, IkappaB prevents nuclear translocation and DNA binding of p65 by masking its nuclear localization signal.	bind
46613	6	7034	6	13	NULL	NULL	NULL	p65	GP		complex with					p105/50	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_21_2707_s_19	12438297	2 In the stable trimeric complex of p65, p105/50, and IkappaB, IkappaB prevents nuclear translocation and DNA binding of p65 by masking its nuclear localization signal.	bind
46614	7	7034	6	13	NULL	NULL	NULL	IkappaB	GP		complex with					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_21_2707_s_19	12438297	2 In the stable trimeric complex of p65, p105/50, and IkappaB, IkappaB prevents nuclear translocation and DNA binding of p65 by masking its nuclear localization signal.	bind
53267	8	7034	6	13	NULL	NULL	NULL	statement 5	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_21_2707_s_19	12438297	2 In the stable trimeric complex of p65, p105/50, and IkappaB, IkappaB prevents nuclear translocation and DNA binding of p65 by masking its nuclear localization signal.	bind
25619	1	7034	7	NULL	NULL	0	NULL	p65	NULL		complex with	NULL				p105/50	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_21_2707_s_19	12438297	2 In the stable trimeric complex of p65, p105/50, and IkappaB, IkappaB prevents nuclear translocation and DNA binding of p65 by masking its nuclear localization signal.	bind
25620	2	7034	7	NULL	NULL	0	NULL	 IkappaB	NULL		forms trimeric complex with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_21_2707_s_19	12438297	2 In the stable trimeric complex of p65, p105/50, and IkappaB, IkappaB prevents nuclear translocation and DNA binding of p65 by masking its nuclear localization signal.	bind
25621	3	7034	7	10	NULL	0	NULL	IkappaB	NULL		prevents	NULL				statement 7	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_21_2707_s_19	12438297	2 In the stable trimeric complex of p65, p105/50, and IkappaB, IkappaB prevents nuclear translocation and DNA binding of p65 by masking its nuclear localization signal.	bind
25622	4	7034	7	NULL	NULL	0	NULL	p65	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_21_2707_s_19	12438297	2 In the stable trimeric complex of p65, p105/50, and IkappaB, IkappaB prevents nuclear translocation and DNA binding of p65 by masking its nuclear localization signal.	bind
25623	5	7034	7	NULL	NULL	0	NULL	IkappaB	NULL		prevents	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_21_2707_s_19	12438297	2 In the stable trimeric complex of p65, p105/50, and IkappaB, IkappaB prevents nuclear translocation and DNA binding of p65 by masking its nuclear localization signal.	bind
25624	6	7034	7	10	NULL	0	NULL	IkappaB	NULL		masks	NULL				p65	NULL		nuclear localization signal		NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_21_2707_s_19	12438297	2 In the stable trimeric complex of p65, p105/50, and IkappaB, IkappaB prevents nuclear translocation and DNA binding of p65 by masking its nuclear localization signal.	bind
53268	7	7034	7	10	NULL	0	NULL	p65	NULL		is translocated to	NULL				nucleus	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_21_2707_s_19	12438297	2 In the stable trimeric complex of p65, p105/50, and IkappaB, IkappaB prevents nuclear translocation and DNA binding of p65 by masking its nuclear localization signal.	bind
53269	8	7034	7	10	NULL	0	NULL	statement 6	NULL		leads to	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_21_2707_s_19	12438297	2 In the stable trimeric complex of p65, p105/50, and IkappaB, IkappaB prevents nuclear translocation and DNA binding of p65 by masking its nuclear localization signal.	bind
21361	1	7035	6	13	NULL	NULL	NULL	AKAP9-LIZ fragment	GP		bind					InsP3R1 SII splice variants	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_19375_s_172	14982933	2 In these experiments we found that AKAP9-LIZ fragment binds to both InsP3R1 SII splice variants, but not to the InsP3R2 or InsP3R3 isoforms ( Fig. 4 B).	bind
21362	2	7035	6	13	NULL	NULL	NULL	AKAP9-LIZ fragment	GP		does not bind					InsP3R2 isoforms	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_19375_s_172	14982933	2 In these experiments we found that AKAP9-LIZ fragment binds to both InsP3R1 SII splice variants, but not to the InsP3R2 or InsP3R3 isoforms ( Fig. 4 B).	bind
21363	3	7035	6	13	NULL	NULL	NULL	AKAP9-LIZ fragment	GP		does not bind					InsP3R3 isoform	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_19375_s_172	14982933	2 In these experiments we found that AKAP9-LIZ fragment binds to both InsP3R1 SII splice variants, but not to the InsP3R2 or InsP3R3 isoforms ( Fig. 4 B).	bind
25625	1	7035	7	NULL	NULL	0	NULL	KAP9-LIZ fragment	NULL		binds	NULL				InsP3R1 SII splice variant	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_18_19375_s_172	14982933	2 In these experiments we found that AKAP9-LIZ fragment binds to both InsP3R1 SII splice variants, but not to the InsP3R2 or InsP3R3 isoforms ( Fig. 4 B).	bind
25626	2	7035	7	NULL	NULL	0	NULL	AKAP9-LIZ fragment	NULL		does not bind	NULL				InsP3R2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_18_19375_s_172	14982933	2 In these experiments we found that AKAP9-LIZ fragment binds to both InsP3R1 SII splice variants, but not to the InsP3R2 or InsP3R3 isoforms ( Fig. 4 B).	bind
25627	3	7035	7	NULL	NULL	0	NULL	AKAP9-LIZ fragment	NULL		does not bind	NULL				InsP3R3 isoforms	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_18_19375_s_172	14982933	2 In these experiments we found that AKAP9-LIZ fragment binds to both InsP3R1 SII splice variants, but not to the InsP3R2 or InsP3R3 isoforms ( Fig. 4 B).	bind
21364	1	7036	6	13	NULL	NULL	NULL	Ral-A	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14525_s_27	10329639	2 In this study we report the effect of Ca2+/calmodulin on GTP binding activity of Ral-A.	bind
25628	1	7036	7	NULL	NULL	0	NULL	GTP 	NULL		bind	NULL				Ral-A	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_21_14525_s_27	10329639	2 In this study we report the effect of Ca2+/calmodulin on GTP binding activity of Ral-A.	bind
22171	1	7037	6	13	NULL	NULL	NULL	proteoglycans	GP		bind		may					high affinity	heparin binding domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_30_18932_s_185	9228073	2 Interactions between cell-surface receptors such as proteoglycans, which may bind the high affinity heparin-binding domain, and either of these integrins must, therefore, occur between separated portions of the FN molecule.	bind
22172	2	7037	6	13	NULL	NULL	NULL	proteoglycans	GP		bind					integrins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_30_18932_s_185	9228073	2 Interactions between cell-surface receptors such as proteoglycans, which may bind the high affinity heparin-binding domain, and either of these integrins must, therefore, occur between separated portions of the FN molecule.	bind
23103	3	7037	6	13	NULL	NULL	NULL	proteoglycans	GP		is a type of					cell surface receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_30_18932_s_185	9228073	2 Interactions between cell-surface receptors such as proteoglycans, which may bind the high affinity heparin-binding domain, and either of these integrins must, therefore, occur between separated portions of the FN molecule.	bind
25857	4	7037	6	13	NULL	NULL	NULL	integrins	GP		occur between					FN molecule	GP	separated portions of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_30_18932_s_185	9228073	2 Interactions between cell-surface receptors such as proteoglycans, which may bind the high affinity heparin-binding domain, and either of these integrins must, therefore, occur between separated portions of the FN molecule.	bind
25858	5	7037	6	13	NULL	NULL	NULL	statement 2	Process		occurs via					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_30_18932_s_185	9228073	2 Interactions between cell-surface receptors such as proteoglycans, which may bind the high affinity heparin-binding domain, and either of these integrins must, therefore, occur between separated portions of the FN molecule.	bind
25629	1	7037	7	NULL	NULL	0	NULL	proteoglycans	NULL		bind	NULL	may				NULL	high affinity	heparin-binding domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_30_18932_s_185	9228073	2 Interactions between cell-surface receptors such as proteoglycans, which may bind the high affinity heparin-binding domain, and either of these integrins must, therefore, occur between separated portions of the FN molecule.	bind
25630	2	7037	7	NULL	NULL	0	NULL	proteoglycans	NULL		bind	NULL				integrins	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_30_18932_s_185	9228073	2 Interactions between cell-surface receptors such as proteoglycans, which may bind the high affinity heparin-binding domain, and either of these integrins must, therefore, occur between separated portions of the FN molecule.	bind
25631	3	7037	7	NULL	NULL	0	NULL	statement 2	NULL		occur between	NULL				FN molecule	NULL	separated portions of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_30_18932_s_185	9228073	2 Interactions between cell-surface receptors such as proteoglycans, which may bind the high affinity heparin-binding domain, and either of these integrins must, therefore, occur between separated portions of the FN molecule.	bind
25880	4	7037	7	10	NULL	0	NULL	proteoglycans	NULL		is a type of	NULL				cell-surface receptors	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_30_18932_s_185	9228073	2 Interactions between cell-surface receptors such as proteoglycans, which may bind the high affinity heparin-binding domain, and either of these integrins must, therefore, occur between separated portions of the FN molecule.	bind
22173	1	7038	6	13	NULL	NULL	NULL	clones RD	NucleicAcid		bind		selectively			albumin	GP	rat			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_38_35035_s_247	12119302	2 Interestingly, SA08, a matured sequence derived from libraries patterned after the sequence of the multispecies binding clone RB, inhibited the binding of clones RD and BA, which selectively bound rat and rabbit albumin, respectively.	bind
22174	2	7038	6	13	NULL	NULL	NULL	clones BA	NucleicAcid		bind		selectively			albumin	GP	rabbit			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_38_35035_s_247	12119302	2 Interestingly, SA08, a matured sequence derived from libraries patterned after the sequence of the multispecies binding clone RB, inhibited the binding of clones RD and BA, which selectively bound rat and rabbit albumin, respectively.	bind
22175	3	7038	6	13	NULL	NULL	NULL	SA08	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_38_35035_s_247	12119302	2 Interestingly, SA08, a matured sequence derived from libraries patterned after the sequence of the multispecies binding clone RB, inhibited the binding of clones RD and BA, which selectively bound rat and rabbit albumin, respectively.	bind
22176	4	7038	6	13	NULL	NULL	NULL	SA08	GP		inhibits					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_38_35035_s_247	12119302	2 Interestingly, SA08, a matured sequence derived from libraries patterned after the sequence of the multispecies binding clone RB, inhibited the binding of clones RD and BA, which selectively bound rat and rabbit albumin, respectively.	bind
25632	1	7038	7	NULL	NULL	0	NULL	clones RD	NULL		bind	NULL	selectively			albumin	NULL	rat			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_38_35035_s_247	12119302	2 Interestingly, SA08, a matured sequence derived from libraries patterned after the sequence of the multispecies binding clone RB, inhibited the binding of clones RD and BA, which selectively bound rat and rabbit albumin, respectively.	bind
25633	2	7038	7	NULL	NULL	0	NULL	clones BA	NULL		bind	NULL	selectively			albumin	NULL	rabbit			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_38_35035_s_247	12119302	2 Interestingly, SA08, a matured sequence derived from libraries patterned after the sequence of the multispecies binding clone RB, inhibited the binding of clones RD and BA, which selectively bound rat and rabbit albumin, respectively.	bind
25634	3	7038	7	NULL	NULL	0	NULL	SA08	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_38_35035_s_247	12119302	2 Interestingly, SA08, a matured sequence derived from libraries patterned after the sequence of the multispecies binding clone RB, inhibited the binding of clones RD and BA, which selectively bound rat and rabbit albumin, respectively.	bind
25635	4	7038	7	NULL	NULL	0	NULL	SA08	NULL		inhibits	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_38_35035_s_247	12119302	2 Interestingly, SA08, a matured sequence derived from libraries patterned after the sequence of the multispecies binding clone RB, inhibited the binding of clones RD and BA, which selectively bound rat and rabbit albumin, respectively.	bind
21365	1	7039	6	13	NULL	NULL	NULL	Ce-MAN1	GP		bind					BAF	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_14_13863_s_217	15681850	2 It is noteworthy that the SRV motif is also present in domain D, shared by Ce-MAN1 (data not shown) and human MAN1 (see Figs.  1 and  2 A), which might account for the binding of Ce-MAN1 to BAF.	bind
21366	2	7039	6	13	NULL	NULL	NULL				is shared by			SRV motif		MAN1	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_14_13863_s_217	15681850	2 It is noteworthy that the SRV motif is also present in domain D, shared by Ce-MAN1 (data not shown) and human MAN1 (see Figs.  1 and  2 A), which might account for the binding of Ce-MAN1 to BAF.	bind
27023	3	7039	6	13	NULL	NULL	NULL				is present in			SRV motif					domain D		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_14_13863_s_217	15681850	2 It is noteworthy that the SRV motif is also present in domain D, shared by Ce-MAN1 (data not shown) and human MAN1 (see Figs.  1 and  2 A), which might account for the binding of Ce-MAN1 to BAF.	bind
27024	4	7039	6	13	NULL	NULL	NULL				is shared by			SRV motif		Ce-MAN1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_14_13863_s_217	15681850	2 It is noteworthy that the SRV motif is also present in domain D, shared by Ce-MAN1 (data not shown) and human MAN1 (see Figs.  1 and  2 A), which might account for the binding of Ce-MAN1 to BAF.	bind
25636	1	7039	7	NULL	NULL	0	NULL	Ce-MAN1	NULL		bind	NULL				BAF	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_14_13863_s_217	15681850	2 It is noteworthy that the SRV motif is also present in domain D, shared by Ce-MAN1 (data not shown) and human MAN1 (see Figs.  1 and  2 A), which might account for the binding of Ce-MAN1 to BAF.	bind
25666	2	7039	7	NULL	NULL	0	NULL		NULL		is present in	NULL		SRV motif			NULL		domain D		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_14_13863_s_217	15681850	2 It is noteworthy that the SRV motif is also present in domain D, shared by Ce-MAN1 (data not shown) and human MAN1 (see Figs.  1 and  2 A), which might account for the binding of Ce-MAN1 to BAF.	bind
25667	3	7039	7	NULL	NULL	0	NULL		NULL		is shared by	NULL		SRV motif		Ce-MAN1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_14_13863_s_217	15681850	2 It is noteworthy that the SRV motif is also present in domain D, shared by Ce-MAN1 (data not shown) and human MAN1 (see Figs.  1 and  2 A), which might account for the binding of Ce-MAN1 to BAF.	bind
25668	4	7039	7	NULL	NULL	0	NULL		NULL		is shared by	NULL		SRV motif		MAN1	NULL	human			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_14_13863_s_217	15681850	2 It is noteworthy that the SRV motif is also present in domain D, shared by Ce-MAN1 (data not shown) and human MAN1 (see Figs.  1 and  2 A), which might account for the binding of Ce-MAN1 to BAF.	bind
21367	1	7040	6	13	NULL	NULL	NULL	p120ctn protein	GP	mutant	bind					E-cadherin polypeptides	GP	nonfunctional			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_30_21409_s_245	10409703	2 It is therefore conceivable that these mutant p120ctn proteins bound to the nonfunctional E-cadherin polypeptides could function as dominant-positive (activating) mutants through facilitating dimerization of the mutant E-cadherin.	bind
27025	2	7040	6	13	NULL	NULL	NULL	statement 1	GP		functions as					dominant-positive (activating) mutants	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_30_21409_s_245	10409703	2 It is therefore conceivable that these mutant p120ctn proteins bound to the nonfunctional E-cadherin polypeptides could function as dominant-positive (activating) mutants through facilitating dimerization of the mutant E-cadherin.	bind
27026	3	7040	6	13	NULL	NULL	NULL	statement 1	GP		dimerize					E-cadherin	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_30_21409_s_245	10409703	2 It is therefore conceivable that these mutant p120ctn proteins bound to the nonfunctional E-cadherin polypeptides could function as dominant-positive (activating) mutants through facilitating dimerization of the mutant E-cadherin.	bind
25637	1	7040	7	NULL	NULL	0	NULL	p120ctn protein	NULL	mutant	bind	NULL				E-cadherin polypeptide	NULL	nonfunctional			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21409_s_245	10409703	2 It is therefore conceivable that these mutant p120ctn proteins bound to the nonfunctional E-cadherin polypeptides could function as dominant-positive (activating) mutants through facilitating dimerization of the mutant E-cadherin.	bind
25638	2	7040	7	NULL	NULL	0	NULL	statement 1	NULL		function as	NULL				dominant-positive mutant	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21409_s_245	10409703	2 It is therefore conceivable that these mutant p120ctn proteins bound to the nonfunctional E-cadherin polypeptides could function as dominant-positive (activating) mutants through facilitating dimerization of the mutant E-cadherin.	bind
25639	3	7040	7	NULL	NULL	0	NULL	statement 1	NULL		dimerize	NULL				E-cadherin	NULL	mutant			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_30_21409_s_245	10409703	2 It is therefore conceivable that these mutant p120ctn proteins bound to the nonfunctional E-cadherin polypeptides could function as dominant-positive (activating) mutants through facilitating dimerization of the mutant E-cadherin.	bind
21379	1	7041	6	13	NULL	NULL	NULL	Fas ligand	GP		bind					Fas	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2354_s_144	8999945	2 It is thus possible that apoptosis of spermatogenic cells is induced by the binding of Fas ligand to Fas through interaction between Sertoli cells and spermatogenic cells.	bind
21380	2	7041	6	13	NULL	NULL	NULL	Sertoli cells	Cell		interacts with					spermatogenic cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2354_s_144	8999945	2 It is thus possible that apoptosis of spermatogenic cells is induced by the binding of Fas ligand to Fas through interaction between Sertoli cells and spermatogenic cells.	bind
21384	3	7041	6	13	NULL	NULL	NULL	statement 1	Process		occurs through					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2354_s_144	8999945	2 It is thus possible that apoptosis of spermatogenic cells is induced by the binding of Fas ligand to Fas through interaction between Sertoli cells and spermatogenic cells.	bind
21389	4	7041	6	13	NULL	NULL	NULL	spermatogenic cells	Cell	apoptosis of	is induced by					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2354_s_144	8999945	2 It is thus possible that apoptosis of spermatogenic cells is induced by the binding of Fas ligand to Fas through interaction between Sertoli cells and spermatogenic cells.	bind
25669	1	7041	7	NULL	NULL	0	NULL	Fas ligand	NULL		bind	NULL				Fas	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_4_2354_s_144	8999945	2 It is thus possible that apoptosis of spermatogenic cells is induced by the binding of Fas ligand to Fas through interaction between Sertoli cells and spermatogenic cells.	bind
25670	2	7041	7	NULL	NULL	0	NULL	Sertoli cells	NULL		interacts with	NULL				spermatogenic cells	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_4_2354_s_144	8999945	2 It is thus possible that apoptosis of spermatogenic cells is induced by the binding of Fas ligand to Fas through interaction between Sertoli cells and spermatogenic cells.	bind
25675	3	7041	7	NULL	NULL	0	NULL	statement 1	NULL		occurs through	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_4_2354_s_144	8999945	2 It is thus possible that apoptosis of spermatogenic cells is induced by the binding of Fas ligand to Fas through interaction between Sertoli cells and spermatogenic cells.	bind
25676	4	7041	7	NULL	NULL	0	NULL	statement 1	NULL		induce	NULL				spermatogenic cells	NULL	apoptosis of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_4_2354_s_144	8999945	2 It is thus possible that apoptosis of spermatogenic cells is induced by the binding of Fas ligand to Fas through interaction between Sertoli cells and spermatogenic cells.	bind
21405	1	7042	6	13	NULL	NULL	NULL	p53	GP		bind		may			EGFR	NucleicAcid			p53RE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_41717_s_284	11546792	2 It is, therefore, possible to speculate that binding affinity of p53 and TAp63gamma to the EGFRp53RE is above and below detection at our level, respectively.	bind
21407	2	7042	6	13	NULL	NULL	NULL	TAp63gamma	GP		bind		may			EGFR	NucleicAcid			p53RE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_41717_s_284	11546792	2 It is, therefore, possible to speculate that binding affinity of p53 and TAp63gamma to the EGFRp53RE is above and below detection at our level, respectively.	bind
25688	1	7042	7	NULL	NULL	0	NULL	p53	NULL		bind	NULL	may			EGFR	NULL			p53RE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_41717_s_284	11546792	2 It is, therefore, possible to speculate that binding affinity of p53 and TAp63gamma to the EGFRp53RE is above and below detection at our level, respectively.	bind
25691	2	7042	7	NULL	NULL	0	NULL	TAp63gamma	NULL		bind	NULL	may			EGFR	NULL			p53RE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_41717_s_284	11546792	2 It is, therefore, possible to speculate that binding affinity of p53 and TAp63gamma to the EGFRp53RE is above and below detection at our level, respectively.	bind
21421	1	7043	6	13	NULL	NULL	NULL	PKG	GP		bind					MBS	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_1_597_s_184	14530290	2 It should be noted that all of the constructs of PKG used by Surks  et al. ( ) containing the LZ also contained the coiled-coil domain, and mutations that disrupted the coiled-coil domain of PKGI inhibited binding of PKG and the MBS.	bind
21424	2	7043	6	13	NULL	NULL	NULL	PKGI	GP	mutant	inhibits			coiled coil domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_1_597_s_184	14530290	2 It should be noted that all of the constructs of PKG used by Surks  et al. ( ) containing the LZ also contained the coiled-coil domain, and mutations that disrupted the coiled-coil domain of PKGI inhibited binding of PKG and the MBS.	bind
25692	1	7043	7	NULL	NULL	0	NULL	PKG	NULL		bind	NULL				MBS	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_1_597_s_184	14530290	2 It should be noted that all of the constructs of PKG used by Surks  et al. ( ) containing the LZ also contained the coiled-coil domain, and mutations that disrupted the coiled-coil domain of PKGI inhibited binding of PKG and the MBS.	bind
25696	2	7043	7	NULL	NULL	0	NULL	PKGI	NULL	mutant	inhibits	NULL		coiled-coil domain		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_1_597_s_184	14530290	2 It should be noted that all of the constructs of PKG used by Surks  et al. ( ) containing the LZ also contained the coiled-coil domain, and mutations that disrupted the coiled-coil domain of PKGI inhibited binding of PKG and the MBS.	bind
21429	1	7044	6	13	NULL	NULL	NULL	h-rhotekin	GP		bind					Rho	GP	active			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_43_33962_s_143	10940294	2 It was also verified that h-rhotekin indeed binds to the active form of Rho.	bind
25697	1	7044	7	NULL	NULL	0	NULL	h-rhotekin	NULL		binds to	NULL				Rho	NULL	active			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_43_33962_s_143	10940294	2 It was also verified that h-rhotekin indeed binds to the active form of Rho.	bind
22177	1	7045	6	13	NULL	NULL	NULL	PDP1c	GP	alone	does not interact		directly			Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_14976_s_361	11842080	2 ITC studies indicate that neither PDP1c nor L2, alone, directly interact with <100 muM Ca2+ and ITC, analytical ultracentrifugation, and other studies indicate L2 and PDP1c bind each in forming a tight Ca2+ binding site ( Kd < 3 muM); similar complex formation by PDP1 is enhanced by Mg2+ (A. Turkan, Y. Hiromasa, and T. E. Roche, manuscript in preparation).	bind
22178	2	7045	6	13	NULL	NULL	NULL	L2	GP	alone	does not interact		directly			Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_14976_s_361	11842080	2 ITC studies indicate that neither PDP1c nor L2, alone, directly interact with <100 muM Ca2+ and ITC, analytical ultracentrifugation, and other studies indicate L2 and PDP1c bind each in forming a tight Ca2+ binding site ( Kd < 3 muM); similar complex formation by PDP1 is enhanced by Mg2+ (A. Turkan, Y. Hiromasa, and T. E. Roche, manuscript in preparation).	bind
22179	3	7045	6	13	NULL	NULL	NULL	PDP1c	GP		bind					L2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_14976_s_361	11842080	2 ITC studies indicate that neither PDP1c nor L2, alone, directly interact with <100 muM Ca2+ and ITC, analytical ultracentrifugation, and other studies indicate L2 and PDP1c bind each in forming a tight Ca2+ binding site ( Kd < 3 muM); similar complex formation by PDP1 is enhanced by Mg2+ (A. Turkan, Y. Hiromasa, and T. E. Roche, manuscript in preparation).	bind
22180	4	7045	6	13	NULL	NULL	NULL	statement 3	Process		forms a								Ca2+ binding site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_14976_s_361	11842080	2 ITC studies indicate that neither PDP1c nor L2, alone, directly interact with <100 muM Ca2+ and ITC, analytical ultracentrifugation, and other studies indicate L2 and PDP1c bind each in forming a tight Ca2+ binding site ( Kd < 3 muM); similar complex formation by PDP1 is enhanced by Mg2+ (A. Turkan, Y. Hiromasa, and T. E. Roche, manuscript in preparation).	bind
22181	5	7045	6	13	NULL	NULL	NULL	PDP1	GP	complex formation by	is enhanced by					Mg2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_14976_s_361	11842080	2 ITC studies indicate that neither PDP1c nor L2, alone, directly interact with <100 muM Ca2+ and ITC, analytical ultracentrifugation, and other studies indicate L2 and PDP1c bind each in forming a tight Ca2+ binding site ( Kd < 3 muM); similar complex formation by PDP1 is enhanced by Mg2+ (A. Turkan, Y. Hiromasa, and T. E. Roche, manuscript in preparation).	bind
53302	6	7045	6	13	NULL	NULL	NULL	PDP1c	GP	alone	does not bind		directly			ITC	ResearchActivity				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_14976_s_361	11842080	2 ITC studies indicate that neither PDP1c nor L2, alone, directly interact with <100 muM Ca2+ and ITC, analytical ultracentrifugation, and other studies indicate L2 and PDP1c bind each in forming a tight Ca2+ binding site ( Kd < 3 muM); similar complex formation by PDP1 is enhanced by Mg2+ (A. Turkan, Y. Hiromasa, and T. E. Roche, manuscript in preparation).	bind
53303	7	7045	6	13	NULL	NULL	NULL	L2	GP	alone	does not bind		directly			ITC	ResearchActivity				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_14976_s_361	11842080	2 ITC studies indicate that neither PDP1c nor L2, alone, directly interact with <100 muM Ca2+ and ITC, analytical ultracentrifugation, and other studies indicate L2 and PDP1c bind each in forming a tight Ca2+ binding site ( Kd < 3 muM); similar complex formation by PDP1 is enhanced by Mg2+ (A. Turkan, Y. Hiromasa, and T. E. Roche, manuscript in preparation).	bind
25698	1	7045	7	10	NULL	0	NULL	PDP1c 	NULL	alone	does not interact with	NULL	directly			Ca2+	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_14976_s_361	11842080	2 ITC studies indicate that neither PDP1c nor L2, alone, directly interact with <100 muM Ca2+ and ITC, analytical ultracentrifugation, and other studies indicate L2 and PDP1c bind each in forming a tight Ca2+ binding site ( Kd < 3 muM); similar complex formation by PDP1 is enhanced by Mg2+ (A. Turkan, Y. Hiromasa, and T. E. Roche, manuscript in preparation).	bind
25699	2	7045	7	10	NULL	0	NULL	L2	NULL	alone	does not interact with	NULL	directly			Ca2+	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_14976_s_361	11842080	2 ITC studies indicate that neither PDP1c nor L2, alone, directly interact with <100 muM Ca2+ and ITC, analytical ultracentrifugation, and other studies indicate L2 and PDP1c bind each in forming a tight Ca2+ binding site ( Kd < 3 muM); similar complex formation by PDP1 is enhanced by Mg2+ (A. Turkan, Y. Hiromasa, and T. E. Roche, manuscript in preparation).	bind
25701	3	7045	7	10	NULL	0	NULL	PDP1c 	NULL	alone	does not interact with	NULL	directly			ITC	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_14976_s_361	11842080	2 ITC studies indicate that neither PDP1c nor L2, alone, directly interact with <100 muM Ca2+ and ITC, analytical ultracentrifugation, and other studies indicate L2 and PDP1c bind each in forming a tight Ca2+ binding site ( Kd < 3 muM); similar complex formation by PDP1 is enhanced by Mg2+ (A. Turkan, Y. Hiromasa, and T. E. Roche, manuscript in preparation).	bind
25702	4	7045	7	10	NULL	0	NULL	L2	NULL	alone	does not interact with	NULL	directly			ITC	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_14976_s_361	11842080	2 ITC studies indicate that neither PDP1c nor L2, alone, directly interact with <100 muM Ca2+ and ITC, analytical ultracentrifugation, and other studies indicate L2 and PDP1c bind each in forming a tight Ca2+ binding site ( Kd < 3 muM); similar complex formation by PDP1 is enhanced by Mg2+ (A. Turkan, Y. Hiromasa, and T. E. Roche, manuscript in preparation).	bind
25703	5	7045	7	NULL	NULL	0	NULL	L2	NULL		bind	NULL				PDP1c 	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_17_14976_s_361	11842080	2 ITC studies indicate that neither PDP1c nor L2, alone, directly interact with <100 muM Ca2+ and ITC, analytical ultracentrifugation, and other studies indicate L2 and PDP1c bind each in forming a tight Ca2+ binding site ( Kd < 3 muM); similar complex formation by PDP1 is enhanced by Mg2+ (A. Turkan, Y. Hiromasa, and T. E. Roche, manuscript in preparation).	bind
25704	6	7045	7	NULL	NULL	0	NULL	statement 5	NULL		forms	NULL				Ca2+	NULL	tight binding site for			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_14976_s_361	11842080	2 ITC studies indicate that neither PDP1c nor L2, alone, directly interact with <100 muM Ca2+ and ITC, analytical ultracentrifugation, and other studies indicate L2 and PDP1c bind each in forming a tight Ca2+ binding site ( Kd < 3 muM); similar complex formation by PDP1 is enhanced by Mg2+ (A. Turkan, Y. Hiromasa, and T. E. Roche, manuscript in preparation).	bind
25705	7	7045	7	10	NULL	0	NULL	Mg2+	NULL		enhance	NULL				PDP1	NULL	complex formation by			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_14976_s_361	11842080	2 ITC studies indicate that neither PDP1c nor L2, alone, directly interact with <100 muM Ca2+ and ITC, analytical ultracentrifugation, and other studies indicate L2 and PDP1c bind each in forming a tight Ca2+ binding site ( Kd < 3 muM); similar complex formation by PDP1 is enhanced by Mg2+ (A. Turkan, Y. Hiromasa, and T. E. Roche, manuscript in preparation).	bind
21435	1	7046	6	13	NULL	NULL	NULL	AP-1	GP		exhibits					TF binding activity	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_13_8558_s_119	9079686	2 Likewise, forskolin partially suppressed TF binding activities of AP-1 and NUR-77 induced by alphaCD3 (Fig.  2 B).	bind
21436	2	7046	6	13	NULL	NULL	NULL	NUR-77	GP		exhibits					TF binding activity	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_13_8558_s_119	9079686	2 Likewise, forskolin partially suppressed TF binding activities of AP-1 and NUR-77 induced by alphaCD3 (Fig.  2 B).	bind
21437	3	7046	6	13	NULL	NULL	NULL	alphaCD3	GP		induces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_13_8558_s_119	9079686	2 Likewise, forskolin partially suppressed TF binding activities of AP-1 and NUR-77 induced by alphaCD3 (Fig.  2 B).	bind
21439	4	7046	6	13	NULL	NULL	NULL	alphaCD3	GP		induces					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_13_8558_s_119	9079686	2 Likewise, forskolin partially suppressed TF binding activities of AP-1 and NUR-77 induced by alphaCD3 (Fig.  2 B).	bind
21443	5	7046	6	13	NULL	NULL	NULL	forskolin	Chemical		suppress		partially			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_13_8558_s_119	9079686	2 Likewise, forskolin partially suppressed TF binding activities of AP-1 and NUR-77 induced by alphaCD3 (Fig.  2 B).	bind
21444	6	7046	6	13	NULL	NULL	NULL	forskolin	Chemical		suppress		partially			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_13_8558_s_119	9079686	2 Likewise, forskolin partially suppressed TF binding activities of AP-1 and NUR-77 induced by alphaCD3 (Fig.  2 B).	bind
25706	2	7046	7	10	NULL	0	NULL	alphaCD3	NULL		induce	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_13_8558_s_119	9079686	2 Likewise, forskolin partially suppressed TF binding activities of AP-1 and NUR-77 induced by alphaCD3 (Fig.  2 B).	bind
25707	4	7046	7	10	NULL	0	NULL	alphaCD3	NULL		induce	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_13_8558_s_119	9079686	2 Likewise, forskolin partially suppressed TF binding activities of AP-1 and NUR-77 induced by alphaCD3 (Fig.  2 B).	bind
25708	5	7046	7	10	NULL	0	NULL	forskolin	NULL		suppress	NULL	partially			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_13_8558_s_119	9079686	2 Likewise, forskolin partially suppressed TF binding activities of AP-1 and NUR-77 induced by alphaCD3 (Fig.  2 B).	bind
25709	6	7046	7	10	NULL	0	NULL	forskolin	NULL		suppress	NULL	partially			statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_13_8558_s_119	9079686	2 Likewise, forskolin partially suppressed TF binding activities of AP-1 and NUR-77 induced by alphaCD3 (Fig.  2 B).	bind
46416	1	7046	7	10	NULL	0	NULL	AP-1	NULL		exhibits	NULL				TF binding activity	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_13_8558_s_119	9079686	2 Likewise, forskolin partially suppressed TF binding activities of AP-1 and NUR-77 induced by alphaCD3 (Fig.  2 B).	bind
46417	3	7046	7	10	NULL	0	NULL	NUR-77	NULL		exhibits	NULL				TF binding activity	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_13_8558_s_119	9079686	2 Likewise, forskolin partially suppressed TF binding activities of AP-1 and NUR-77 induced by alphaCD3 (Fig.  2 B).	bind
21554	1	7047	6	13	NULL	NULL	NULL	RasGRP1.2	GP		is localized in					endoplasmic reticulum	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_35_33465_s_309	12782630	2 Likewise, treatment of cells with a phospholipase Cgamma chemical inhibitor  does not abolish the reticular distribution of RasGRP1.2 Based on  those results, we surmise that the localization of RasGRP1 in the endoplasmic  reticulum is helped by the binding of the RasGRP1 ZF to a docking protein  present in that subcellular compartment.	bind
21555	2	7047	6	13	NULL	NULL	NULL	RasGRP1	GP		bind			ZF		docking protein	GP				NULL	subcellular compartment	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_35_33465_s_309	12782630	2 Likewise, treatment of cells with a phospholipase Cgamma chemical inhibitor  does not abolish the reticular distribution of RasGRP1.2 Based on  those results, we surmise that the localization of RasGRP1 in the endoplasmic  reticulum is helped by the binding of the RasGRP1 ZF to a docking protein  present in that subcellular compartment.	bind
21556	3	7047	6	13	NULL	NULL	NULL	phospholipase Cgamma	GP		does not abolish					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_35_33465_s_309	12782630	2 Likewise, treatment of cells with a phospholipase Cgamma chemical inhibitor  does not abolish the reticular distribution of RasGRP1.2 Based on  those results, we surmise that the localization of RasGRP1 in the endoplasmic  reticulum is helped by the binding of the RasGRP1 ZF to a docking protein  present in that subcellular compartment.	bind
46418	4	7047	6	13	NULL	NULL	NULL	\tphospholipase Cgamma	GP		is a type of					chemical inhibitor					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_35_33465_s_309	12782630	2 Likewise, treatment of cells with a phospholipase Cgamma chemical inhibitor  does not abolish the reticular distribution of RasGRP1.2 Based on  those results, we surmise that the localization of RasGRP1 in the endoplasmic  reticulum is helped by the binding of the RasGRP1 ZF to a docking protein  present in that subcellular compartment.	bind
25710	2	7047	7	10	NULL	0	NULL	phospholipase Cgamma 	NULL		does not abolish	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_35_33465_s_309	12782630	2 Likewise, treatment of cells with a phospholipase Cgamma chemical inhibitor  does not abolish the reticular distribution of RasGRP1.2 Based on  those results, we surmise that the localization of RasGRP1 in the endoplasmic  reticulum is helped by the binding of the RasGRP1 ZF to a docking protein  present in that subcellular compartment.	bind
25711	3	7047	7	10	NULL	0	NULL	RasGRP1	NULL		bind	NULL		ZF		docking protein	NULL				NULL	subcellular compartment	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_35_33465_s_309	12782630	2 Likewise, treatment of cells with a phospholipase Cgamma chemical inhibitor  does not abolish the reticular distribution of RasGRP1.2 Based on  those results, we surmise that the localization of RasGRP1 in the endoplasmic  reticulum is helped by the binding of the RasGRP1 ZF to a docking protein  present in that subcellular compartment.	bind
25713	4	7047	7	10	NULL	0	NULL	statement 3	NULL		helps	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_35_33465_s_309	12782630	2 Likewise, treatment of cells with a phospholipase Cgamma chemical inhibitor  does not abolish the reticular distribution of RasGRP1.2 Based on  those results, we surmise that the localization of RasGRP1 in the endoplasmic  reticulum is helped by the binding of the RasGRP1 ZF to a docking protein  present in that subcellular compartment.	bind
46419	1	7047	7	10	NULL	0	NULL	RasGRP1	NULL		is localized in	NULL				endoplasmic reticulum	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_35_33465_s_309	12782630	2 Likewise, treatment of cells with a phospholipase Cgamma chemical inhibitor  does not abolish the reticular distribution of RasGRP1.2 Based on  those results, we surmise that the localization of RasGRP1 in the endoplasmic  reticulum is helped by the binding of the RasGRP1 ZF to a docking protein  present in that subcellular compartment.	bind
21560	1	7048	6	13	NULL	NULL	NULL	ACP	GP		bind					Glycerol	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_1_194_s_63	12409302	2 M glycerol, suggesting that ACP binds glycerol.	bind
25715	1	7048	7	NULL	NULL	0	NULL	ACP	NULL		binds	NULL				glycerol	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_1_194_s_63	12409302	2 M glycerol, suggesting that ACP binds glycerol.	bind
21561	1	7049	6	13	NULL	NULL	NULL	mAb 1E5	GP		bind		specifically			BP230	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_16_9711_s_44	9545306	2 mAb 1E5 binds specifically to BP230.	bind
25716	1	7049	7	NULL	NULL	0	NULL	mAb 1E5	NULL		bind	NULL	specifically			BP230	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_16_9711_s_44	9545306	2 mAb 1E5 binds specifically to BP230.	bind
21562	1	7050	6	13	NULL	NULL	NULL	CD4	GP		bind					mAb	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_508_1_67_s_113	11707270	2 mAb demonstrating CD4 binding ability	bind
25882	1	7050	7	NULL	NULL	0	NULL	mAb	NULL		binds	NULL				CD4	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_508_1_67_s_113	11707270	2 mAb demonstrating CD4 binding ability	bind
21563	1	7051	6	13	NULL	NULL	NULL	nonO	GP		contain		may			CA enzymatic activity	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_16044_s_136	10821857	2 mM acetazolamide completely prevented the binding of both nonO and CA II to the column, suggesting that the binding properties of nonO and CA II are quite similar and that nonO may also contain CA enzymatic activity.	bind
21571	2	7051	6	13	NULL	NULL	NULL	nonO	GP	binding properties of	are quite similar to					CA II	GP	binding properties of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_16044_s_136	10821857	2 mM acetazolamide completely prevented the binding of both nonO and CA II to the column, suggesting that the binding properties of nonO and CA II are quite similar and that nonO may also contain CA enzymatic activity.	bind
25717	1	7051	7	NULL	NULL	0	NULL	nonO	NULL		contain	NULL	may			CA enzymatic activity	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_16044_s_136	10821857	2 mM acetazolamide completely prevented the binding of both nonO and CA II to the column, suggesting that the binding properties of nonO and CA II are quite similar and that nonO may also contain CA enzymatic activity.	bind
25881	2	7051	7	NULL	NULL	0	NULL	nonO	NULL	 binding properties of 	are quite similar to	NULL				CA II	NULL	binding properties of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_16044_s_136	10821857	2 mM acetazolamide completely prevented the binding of both nonO and CA II to the column, suggesting that the binding properties of nonO and CA II are quite similar and that nonO may also contain CA enzymatic activity.	bind
21574	1	7053	6	13	NULL	NULL	NULL	calmodulin	GP	biotinylated	bind					Ral-A	GP	renatured			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_25_16002_s_229	9188503	2 Moreover, biotinylated calmodulin overlay experiments have shown that biotinylated calmodulin binds to renatured Ral-A in a Ca2+-dependent manner, confirming our finding that Ral-A is a calmodulin-binding protein.	bind
21575	2	7053	6	13	NULL	NULL	NULL	statement 1	Process		is dependent on					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_25_16002_s_229	9188503	2 Moreover, biotinylated calmodulin overlay experiments have shown that biotinylated calmodulin binds to renatured Ral-A in a Ca2+-dependent manner, confirming our finding that Ral-A is a calmodulin-binding protein.	bind
21576	3	7053	6	13	NULL	NULL	NULL	Ral-A	GP		is a type of					calmodulin-binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_25_16002_s_229	9188503	2 Moreover, biotinylated calmodulin overlay experiments have shown that biotinylated calmodulin binds to renatured Ral-A in a Ca2+-dependent manner, confirming our finding that Ral-A is a calmodulin-binding protein.	bind
25719	1	7053	7	NULL	NULL	0	NULL	calmodulin	NULL	biotinylated	binds to	NULL				Ral-A	NULL	renatured 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_25_16002_s_229	9188503	2 Moreover, biotinylated calmodulin overlay experiments have shown that biotinylated calmodulin binds to renatured Ral-A in a Ca2+-dependent manner, confirming our finding that Ral-A is a calmodulin-binding protein.	bind
25720	2	7053	7	NULL	NULL	0	NULL	statement 1	NULL		depends on	NULL				Ca2+	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_25_16002_s_229	9188503	2 Moreover, biotinylated calmodulin overlay experiments have shown that biotinylated calmodulin binds to renatured Ral-A in a Ca2+-dependent manner, confirming our finding that Ral-A is a calmodulin-binding protein.	bind
25721	3	7053	7	NULL	NULL	0	NULL	Ral-A	NULL		is a type of	NULL				calmodulin-binding protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_25_16002_s_229	9188503	2 Moreover, biotinylated calmodulin overlay experiments have shown that biotinylated calmodulin binds to renatured Ral-A in a Ca2+-dependent manner, confirming our finding that Ral-A is a calmodulin-binding protein.	bind
22182	1	7058	6	13	NULL	NULL	NULL	caldesmon	GP		is located between		primarily	myosin binding domain					residues 25 and 53		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3213_s_234	10652307	2 MY27C binds less strongly2 and was less potent and less effective in the present study, consistent with the myosin binding domain of caldesmon being primarily located between residues 25 and 53, but also, to a lesser extent, extending to the N terminus.	bind
22183	2	7058	6	13	NULL	NULL	NULL	caldesmon	GP		is extended to 			myosin binding domain					N-terminus		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3213_s_234	10652307	2 MY27C binds less strongly2 and was less potent and less effective in the present study, consistent with the myosin binding domain of caldesmon being primarily located between residues 25 and 53, but also, to a lesser extent, extending to the N terminus.	bind
21591	1	7059	6	13	NULL	NULL	NULL	scuPA	GP		forms a complex with					sDI	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_5348_s_171	9030610	2 Nevertheless, the observation that complexes composed of scuPA and sDI, sDII-DIII, or full-length suPAR bind to LMTK  cells to the same extent provides additional support for the involvement of urokinase in this interaction.	bind
21592	2	7059	6	13	NULL	NULL	NULL	statement 1	GP		forms a complex with					sDII-DIII	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_5348_s_171	9030610	2 Nevertheless, the observation that complexes composed of scuPA and sDI, sDII-DIII, or full-length suPAR bind to LMTK  cells to the same extent provides additional support for the involvement of urokinase in this interaction.	bind
21593	3	7059	6	13	NULL	NULL	NULL	statement 1	GP		forms a complex with					suPAR	GP	full length			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_5348_s_171	9030610	2 Nevertheless, the observation that complexes composed of scuPA and sDI, sDII-DIII, or full-length suPAR bind to LMTK  cells to the same extent provides additional support for the involvement of urokinase in this interaction.	bind
21594	4	7059	6	13	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_5348_s_171	9030610	2 Nevertheless, the observation that complexes composed of scuPA and sDI, sDII-DIII, or full-length suPAR bind to LMTK  cells to the same extent provides additional support for the involvement of urokinase in this interaction.	bind
21595	5	7059	6	13	NULL	NULL	NULL	statement 3	GP		bind					LMTK cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_5348_s_171	9030610	2 Nevertheless, the observation that complexes composed of scuPA and sDI, sDII-DIII, or full-length suPAR bind to LMTK  cells to the same extent provides additional support for the involvement of urokinase in this interaction.	bind
22184	6	7059	6	13	NULL	NULL	NULL	statement 2	GP		bind					LMTK cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_5348_s_171	9030610	2 Nevertheless, the observation that complexes composed of scuPA and sDI, sDII-DIII, or full-length suPAR bind to LMTK  cells to the same extent provides additional support for the involvement of urokinase in this interaction.	bind
22185	7	7059	6	13	NULL	NULL	NULL	urokinase	GP		is involved in					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_5348_s_171	9030610	2 Nevertheless, the observation that complexes composed of scuPA and sDI, sDII-DIII, or full-length suPAR bind to LMTK  cells to the same extent provides additional support for the involvement of urokinase in this interaction.	bind
22186	8	7059	6	13	NULL	NULL	NULL	urokinase	GP		is involved in					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_5348_s_171	9030610	2 Nevertheless, the observation that complexes composed of scuPA and sDI, sDII-DIII, or full-length suPAR bind to LMTK  cells to the same extent provides additional support for the involvement of urokinase in this interaction.	bind
25885	1	7059	7	NULL	NULL	0	NULL	scuPA	NULL		forms complex with	NULL				sDI	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_8_5348_s_171	9030610	2 Nevertheless, the observation that complexes composed of scuPA and sDI, sDII-DIII, or full-length suPAR bind to LMTK  cells to the same extent provides additional support for the involvement of urokinase in this interaction.	bind
25886	2	7059	7	NULL	NULL	0	NULL	statement 1			forms complex with					sDII-DIII					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_5348_s_171	9030610	2 Nevertheless, the observation that complexes composed of scuPA and sDI, sDII-DIII, or full-length suPAR bind to LMTK  cells to the same extent provides additional support for the involvement of urokinase in this interaction.	bind
25887	3	7059	7	NULL	NULL	0	NULL	statement 1			forms complex with					suPAR		full-length			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_5348_s_171	9030610	2 Nevertheless, the observation that complexes composed of scuPA and sDI, sDII-DIII, or full-length suPAR bind to LMTK  cells to the same extent provides additional support for the involvement of urokinase in this interaction.	bind
25888	4	7059	7	NULL	NULL	0	NULL	statement 2			bind					LMTK cells					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_5348_s_171	9030610	2 Nevertheless, the observation that complexes composed of scuPA and sDI, sDII-DIII, or full-length suPAR bind to LMTK  cells to the same extent provides additional support for the involvement of urokinase in this interaction.	bind
25889	5	7059	7	NULL	NULL	0	NULL	statement 3			bind					LMTK cells					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_5348_s_171	9030610	2 Nevertheless, the observation that complexes composed of scuPA and sDI, sDII-DIII, or full-length suPAR bind to LMTK  cells to the same extent provides additional support for the involvement of urokinase in this interaction.	bind
25890	6	7059	7	NULL	NULL	0	NULL	statement 2			is an alternative to					statement 3					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_5348_s_171	9030610	2 Nevertheless, the observation that complexes composed of scuPA and sDI, sDII-DIII, or full-length suPAR bind to LMTK  cells to the same extent provides additional support for the involvement of urokinase in this interaction.	bind
25891	7	7059	7	NULL	NULL	0	NULL	urokinase			is involved in					statement 4					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_5348_s_171	9030610	2 Nevertheless, the observation that complexes composed of scuPA and sDI, sDII-DIII, or full-length suPAR bind to LMTK  cells to the same extent provides additional support for the involvement of urokinase in this interaction.	bind
25892	8	7059	7	NULL	NULL	0	NULL	urokinase			is involved in					statement 5					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_5348_s_171	9030610	2 Nevertheless, the observation that complexes composed of scuPA and sDI, sDII-DIII, or full-length suPAR bind to LMTK  cells to the same extent provides additional support for the involvement of urokinase in this interaction.	bind
21598	1	7060	6	13	NULL	NULL	NULL	TRAF	GP		bind					CD40	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_19777_s_124	9242637	2 NF-kappaB activation is also a major function associated with TRAF binding to TNF receptor family members including CD40.	bind
21599	2	7060	6	13	NULL	NULL	NULL	CD40	GP		is a type of					TNF receptor family members	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_19777_s_124	9242637	2 NF-kappaB activation is also a major function associated with TRAF binding to TNF receptor family members including CD40.	bind
21601	3	7060	6	13	NULL	NULL	NULL	NF-kappaB 	GP	activation of	is associated with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_19777_s_124	9242637	2 NF-kappaB activation is also a major function associated with TRAF binding to TNF receptor family members including CD40.	bind
25897	1	7060	7	NULL	NULL	0	NULL	TRAF	NULL		bind	NULL				CD40	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_32_19777_s_124	9242637	2 NF-kappaB activation is also a major function associated with TRAF binding to TNF receptor family members including CD40.	bind
25898	2	7060	7	NULL	NULL	0	NULL	CD40	NULL		is a type of	NULL				 TNF receptor family	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_32_19777_s_124	9242637	2 NF-kappaB activation is also a major function associated with TRAF binding to TNF receptor family members including CD40.	bind
25899	3	7060	7	10	NULL	0	NULL	NF-kappaB	NULL	activation of	is associated with	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_19777_s_124	9242637	2 NF-kappaB activation is also a major function associated with TRAF binding to TNF receptor family members including CD40.	bind
21810	1	7062	6	13	NULL	NULL	NULL	GRP-R	GP		bind					bombesin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17405_s_16	9211882	2 Notably, GRP-R, NMB-R, and bb4 all bind bombesin with affinities in the nanomolar range, whereas BRS-3 binds bombesin with much lower affinity (>10 muM).	bind
21811	2	7062	6	13	NULL	NULL	NULL	NMB-R	GP		bind					bombesin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17405_s_16	9211882	2 Notably, GRP-R, NMB-R, and bb4 all bind bombesin with affinities in the nanomolar range, whereas BRS-3 binds bombesin with much lower affinity (>10 muM).	bind
21812	3	7062	6	13	NULL	NULL	NULL	bb4	GP		bind					bombesin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17405_s_16	9211882	2 Notably, GRP-R, NMB-R, and bb4 all bind bombesin with affinities in the nanomolar range, whereas BRS-3 binds bombesin with much lower affinity (>10 muM).	bind
21814	4	7062	6	13	NULL	NULL	NULL	BRS-3	GP		bind		low affinity			bombesin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17405_s_16	9211882	2 Notably, GRP-R, NMB-R, and bb4 all bind bombesin with affinities in the nanomolar range, whereas BRS-3 binds bombesin with much lower affinity (>10 muM).	bind
25900	1	7062	7	NULL	NULL	0	NULL	GRP-R	NULL		bind	NULL				bombesin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_28_17405_s_16	9211882	2 Notably, GRP-R, NMB-R, and bb4 all bind bombesin with affinities in the nanomolar range, whereas BRS-3 binds bombesin with much lower affinity (>10 muM).	bind
25901	2	7062	7	NULL	NULL	0	NULL	NMB-R	NULL		bind	NULL				bombesin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_28_17405_s_16	9211882	2 Notably, GRP-R, NMB-R, and bb4 all bind bombesin with affinities in the nanomolar range, whereas BRS-3 binds bombesin with much lower affinity (>10 muM).	bind
25902	3	7062	7	NULL	NULL	0	NULL	bb4	NULL		bind	NULL				bombesin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_28_17405_s_16	9211882	2 Notably, GRP-R, NMB-R, and bb4 all bind bombesin with affinities in the nanomolar range, whereas BRS-3 binds bombesin with much lower affinity (>10 muM).	bind
25903	4	7062	7	NULL	NULL	0	NULL	BRS-3	NULL		bind	NULL	low affinity			bombesin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_28_17405_s_16	9211882	2 Notably, GRP-R, NMB-R, and bb4 all bind bombesin with affinities in the nanomolar range, whereas BRS-3 binds bombesin with much lower affinity (>10 muM).	bind
21820	1	7063	6	13	NULL	NULL	NULL	IgE	GP		bind					fast omega-gliadin	Chemical				NULL	sera of patients with WDEIA	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_13_12135_s_141	14699123	2 of the 15 patients with WDEIA (patients 11 and 13) had no specific IgE bound to these epitopes ( Fig. 5), although their sera had IgE bound to fast omega-gliadin.	bind
25904	1	7063	7	10	NULL	0	NULL	IgE	NULL		bind	NULL				fast omega-gliadin	NULL				NULL	sera of patients with WDEIA	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_13_12135_s_141	14699123	2 of the 15 patients with WDEIA (patients 11 and 13) had no specific IgE bound to these epitopes ( Fig. 5), although their sera had IgE bound to fast omega-gliadin.	bind
21821	1	7064	6	13	NULL	NULL	NULL	MCP-1	GP		bind					CCR2	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_969_s_19	12067906	2 One of the chemoattractants implicated in the early atherogenesis is monocyte chemoattractant protein-1 (MCP-1), which binds to C-C chemokine receptor 2 (CCR2).	bind
21822	2	7064	6	13	NULL	NULL	NULL	MCP-1	GP		is					monocyte chemoattractant protein-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_969_s_19	12067906	2 One of the chemoattractants implicated in the early atherogenesis is monocyte chemoattractant protein-1 (MCP-1), which binds to C-C chemokine receptor 2 (CCR2).	bind
21823	3	7064	6	13	NULL	NULL	NULL	CCR2	GP		is					C-C chemokine receptor 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_969_s_19	12067906	2 One of the chemoattractants implicated in the early atherogenesis is monocyte chemoattractant protein-1 (MCP-1), which binds to C-C chemokine receptor 2 (CCR2).	bind
25905	1	7064	7	NULL	NULL	0	NULL	MCP-1	NULL		binds to	NULL				CCR2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_969_s_19	12067906	2 One of the chemoattractants implicated in the early atherogenesis is monocyte chemoattractant protein-1 (MCP-1), which binds to C-C chemokine receptor 2 (CCR2).	bind
25906	2	7064	7	NULL	NULL	0	NULL	MCP-1	NULL		is	NULL				monocyte chemoattractant protein-1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_969_s_19	12067906	2 One of the chemoattractants implicated in the early atherogenesis is monocyte chemoattractant protein-1 (MCP-1), which binds to C-C chemokine receptor 2 (CCR2).	bind
25907	3	7064	7	NULL	NULL	0	NULL	CCR2	NULL		is	NULL				C-C chemokine receptor 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_969_s_19	12067906	2 One of the chemoattractants implicated in the early atherogenesis is monocyte chemoattractant protein-1 (MCP-1), which binds to C-C chemokine receptor 2 (CCR2).	bind
21907	1	7065	6	13	NULL	NULL	NULL	eIF4G1	GP		bind		directly			eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_30_21297_s_150	10409688	2 Our protease protection data implied that a greater portion of eIF4G1 is directly bound to eIF4E than had been previously supposed and/or that the eIF4E binding domain of eIF4G1 forms a folded structure when the eIF4E binding peptide binds to eIF4E.	bind
21912	2	7065	6	13	NULL	NULL	NULL	eIF4G1	GP		forms a			eIF4E binding domain		folded structure	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_30_21297_s_150	10409688	2 Our protease protection data implied that a greater portion of eIF4G1 is directly bound to eIF4E than had been previously supposed and/or that the eIF4E binding domain of eIF4G1 forms a folded structure when the eIF4E binding peptide binds to eIF4E.	bind
21913	3	7065	6	13	NULL	NULL	NULL	eIF4E binding peptide	GP		bind					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_30_21297_s_150	10409688	2 Our protease protection data implied that a greater portion of eIF4G1 is directly bound to eIF4E than had been previously supposed and/or that the eIF4E binding domain of eIF4G1 forms a folded structure when the eIF4E binding peptide binds to eIF4E.	bind
53304	4	7065	6	13	NULL	NULL	NULL	statement 3	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_30_21297_s_150	10409688	2 Our protease protection data implied that a greater portion of eIF4G1 is directly bound to eIF4E than had been previously supposed and/or that the eIF4E binding domain of eIF4G1 forms a folded structure when the eIF4E binding peptide binds to eIF4E.	bind
25908	1	7065	7	NULL	NULL	0	NULL	eIF4G1	NULL		binds	NULL	directly			eIF4E	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21297_s_150	10409688	2 Our protease protection data implied that a greater portion of eIF4G1 is directly bound to eIF4E than had been previously supposed and/or that the eIF4E binding domain of eIF4G1 forms a folded structure when the eIF4E binding peptide binds to eIF4E.	bind
25909	2	7065	7	NULL	NULL	0	NULL	eIF4G1	NULL		forms a	NULL		eIF4E binding domain 		folded structure	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21297_s_150	10409688	2 Our protease protection data implied that a greater portion of eIF4G1 is directly bound to eIF4E than had been previously supposed and/or that the eIF4E binding domain of eIF4G1 forms a folded structure when the eIF4E binding peptide binds to eIF4E.	bind
25910	3	7065	7	NULL	NULL	0	NULL	eIF4E binding peptide	NULL		binds to	NULL				eIF4E	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21297_s_150	10409688	2 Our protease protection data implied that a greater portion of eIF4G1 is directly bound to eIF4E than had been previously supposed and/or that the eIF4E binding domain of eIF4G1 forms a folded structure when the eIF4E binding peptide binds to eIF4E.	bind
25911	4	7065	7	NULL	NULL	0	NULL	statement 2	NULL		occurs upon	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21297_s_150	10409688	2 Our protease protection data implied that a greater portion of eIF4G1 is directly bound to eIF4E than had been previously supposed and/or that the eIF4E binding domain of eIF4G1 forms a folded structure when the eIF4E binding peptide binds to eIF4E.	bind
21918	1	7066	6	13	NULL	NULL	NULL	GG	NucleicAcid		does not bind		directly			Ras-GRF2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_41_38029_s_225	11500499	2 Overall these results suggest that GG does not bind directly to Ras-GRF2.	bind
25912	1	7066	7	NULL	NULL	0	NULL	 GG	NULL		does not bind	NULL	directly			Ras-GRF2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_41_38029_s_225	11500499	2 Overall these results suggest that GG does not bind directly to Ras-GRF2.	bind
21919	1	7067	6	13	NULL	NULL	NULL	p53	GP		does not bind			His-175		SCS	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_41_25468_s_95	8810317	2 p53(His-175) did not bind to SCS either; however, its generally weaker binding to the other sites makes this observation less significant.	bind
25913	1	7067	7	NULL	NULL	0	NULL	p53	NULL		does not bind	NULL		His-175		SCS	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_41_25468_s_95	8810317	2 p53(His-175) did not bind to SCS either; however, its generally weaker binding to the other sites makes this observation less significant.	bind
21921	1	7069	6	13	NULL	NULL	NULL	F-actin	GP		bind					spinophilin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_2_1186_s_313	12417592	2 Phosphorylation of spinophilin may disrupt one of these sites, reducing the number of actin molecules bound to spinophilin without perturbing the binding affinity of spinophilin for F-actin.	bind
21922	2	7069	6	13	NULL	NULL	NULL	spinophilin	GP	phosphorylation of	reduces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_2_1186_s_313	12417592	2 Phosphorylation of spinophilin may disrupt one of these sites, reducing the number of actin molecules bound to spinophilin without perturbing the binding affinity of spinophilin for F-actin.	bind
21923	3	7069	6	13	NULL	NULL	NULL	spinophilin	GP	phosphorylation of	does not affect					spinophilin	GP	binding affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_2_1186_s_313	12417592	2 Phosphorylation of spinophilin may disrupt one of these sites, reducing the number of actin molecules bound to spinophilin without perturbing the binding affinity of spinophilin for F-actin.	bind
25917	1	7069	7	NULL	NULL	0	NULL	spinophilin	NULL		bind	NULL				F-actin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_2_1186_s_313	12417592	2 Phosphorylation of spinophilin may disrupt one of these sites, reducing the number of actin molecules bound to spinophilin without perturbing the binding affinity of spinophilin for F-actin.	bind
25918	2	7069	7	NULL	NULL	0	NULL	spinophilin	NULL	Phosphorylation of	does not perturb	NULL				statement 1	NULL	binding affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_2_1186_s_313	12417592	2 Phosphorylation of spinophilin may disrupt one of these sites, reducing the number of actin molecules bound to spinophilin without perturbing the binding affinity of spinophilin for F-actin.	bind
25919	3	7069	7	NULL	NULL	0	NULL	spinophilin	NULL	phosphorylation of	reduce	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_2_1186_s_313	12417592	2 Phosphorylation of spinophilin may disrupt one of these sites, reducing the number of actin molecules bound to spinophilin without perturbing the binding affinity of spinophilin for F-actin.	bind
21924	1	7070	6	13	NULL	NULL	NULL	cisplatin	Chemical		bind		rapidly			plasma proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_5_1193_s_316	8636430	2 Previous studies have demonstrated that the large  majority of cisplatin is bound rapidly by plasma proteins, including albumin ( 62).	bind
21925	2	7070	6	13	NULL	NULL	NULL	cisplatin	Chemical		bind					albumin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_5_1193_s_316	8636430	2 Previous studies have demonstrated that the large  majority of cisplatin is bound rapidly by plasma proteins, including albumin ( 62).	bind
27027	3	7070	6	13	NULL	NULL	NULL	albumin	GP		is a type of					plasma protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_5_1193_s_316	8636430	2 Previous studies have demonstrated that the large  majority of cisplatin is bound rapidly by plasma proteins, including albumin ( 62).	bind
25920	1	7070	7	NULL	NULL	0	NULL	cisplatin	NULL		binds	NULL	rapidly			albumin	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_97_5_1193_s_316	8636430	2 Previous studies have demonstrated that the large  majority of cisplatin is bound rapidly by plasma proteins, including albumin ( 62).	bind
25921	2	7070	7	NULL	NULL	0	NULL	albumin	NULL		is a type of	NULL				plasma protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_97_5_1193_s_316	8636430	2 Previous studies have demonstrated that the large  majority of cisplatin is bound rapidly by plasma proteins, including albumin ( 62).	bind
30062	3	7070	7	NULL	NULL	0	NULL	cisplatin	NULL		bind	NULL				plasma proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_97_5_1193_s_316	8636430	2 Previous studies have demonstrated that the large  majority of cisplatin is bound rapidly by plasma proteins, including albumin ( 62).	bind
21926	1	7071	6	13	NULL	NULL	NULL	Axin	GP		bind					beta-catenin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_4_2399_s_76	10644691	2 Previously, it had been shown that Axin binds beta-catenin to regulate its abundance ( 9).	bind
21927	2	7071	6	13	NULL	NULL	NULL	statement 1	Process		regulates					beta-catenin	GP	abundance of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_4_2399_s_76	10644691	2 Previously, it had been shown that Axin binds beta-catenin to regulate its abundance ( 9).	bind
25922	1	7071	7	NULL	NULL	0	NULL	Axin	NULL		binds	NULL				beta-catenin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_4_2399_s_76	10644691	2 Previously, it had been shown that Axin binds beta-catenin to regulate its abundance ( 9).	bind
25923	2	7071	7	NULL	NULL	0	NULL	statement 1	NULL		regulate 	NULL				beta-catenin	NULL	abundance of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_4_2399_s_76	10644691	2 Previously, it had been shown that Axin binds beta-catenin to regulate its abundance ( 9).	bind
21928	1	7072	6	13	NULL	NULL	NULL	JNK	GP		bind					growth factor receptor binding protein 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_38_23304_s_139	8798530	2 Recent studies suggest that JNK binds to growth factor receptor binding protein 2 ( 11), the adapter protein that links tyrosine kinase receptors to the SOS protein, which, in turn, activates p21 ras by promoting GTP/GDP exchange.	bind
21929	2	7072	6	13	NULL	NULL	NULL	tyrosine kinase receptors	GP		linked to					SOS protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_38_23304_s_139	8798530	2 Recent studies suggest that JNK binds to growth factor receptor binding protein 2 ( 11), the adapter protein that links tyrosine kinase receptors to the SOS protein, which, in turn, activates p21 ras by promoting GTP/GDP exchange.	bind
21933	3	7072	6	13	NULL	NULL	NULL	growth factor receptor binding protein 2	GP		plays a role in					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_38_23304_s_139	8798530	2 Recent studies suggest that JNK binds to growth factor receptor binding protein 2 ( 11), the adapter protein that links tyrosine kinase receptors to the SOS protein, which, in turn, activates p21 ras by promoting GTP/GDP exchange.	bind
21935	4	7072	6	13	NULL	NULL	NULL	statement 2	Process		activates					p21 ras	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_38_23304_s_139	8798530	2 Recent studies suggest that JNK binds to growth factor receptor binding protein 2 ( 11), the adapter protein that links tyrosine kinase receptors to the SOS protein, which, in turn, activates p21 ras by promoting GTP/GDP exchange.	bind
21936	5	7072	6	13	NULL	NULL	NULL	statement 4	Process		occurs by					GTP/GDP exchange	Process	promoting 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_38_23304_s_139	8798530	2 Recent studies suggest that JNK binds to growth factor receptor binding protein 2 ( 11), the adapter protein that links tyrosine kinase receptors to the SOS protein, which, in turn, activates p21 ras by promoting GTP/GDP exchange.	bind
27028	6	7072	6	13	NULL	NULL	NULL	growth factor receptor binding protein 2	GP		is a type of					adapter protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_38_23304_s_139	8798530	2 Recent studies suggest that JNK binds to growth factor receptor binding protein 2 ( 11), the adapter protein that links tyrosine kinase receptors to the SOS protein, which, in turn, activates p21 ras by promoting GTP/GDP exchange.	bind
25924	1	7072	7	NULL	NULL	0	NULL	 JNK	NULL		binds to	NULL				growth factor receptor binding protein 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_38_23304_s_139	8798530	2 Recent studies suggest that JNK binds to growth factor receptor binding protein 2 ( 11), the adapter protein that links tyrosine kinase receptors to the SOS protein, which, in turn, activates p21 ras by promoting GTP/GDP exchange.	bind
25925	2	7072	7	NULL	NULL	0	NULL	growth factor receptor binding protein 2	NULL		is a type of	NULL				adaptor protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_38_23304_s_139	8798530	2 Recent studies suggest that JNK binds to growth factor receptor binding protein 2 ( 11), the adapter protein that links tyrosine kinase receptors to the SOS protein, which, in turn, activates p21 ras by promoting GTP/GDP exchange.	bind
25926	3	7072	7	10	NULL	0	NULL	tyrosine kinase receptors	NULL		is linked to	NULL				SOS protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_38_23304_s_139	8798530	2 Recent studies suggest that JNK binds to growth factor receptor binding protein 2 ( 11), the adapter protein that links tyrosine kinase receptors to the SOS protein, which, in turn, activates p21 ras by promoting GTP/GDP exchange.	bind
25927	4	7072	7	10	NULL	0	NULL	growth factor receptor binding protein 2	NULL		plays a role in	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_38_23304_s_139	8798530	2 Recent studies suggest that JNK binds to growth factor receptor binding protein 2 ( 11), the adapter protein that links tyrosine kinase receptors to the SOS protein, which, in turn, activates p21 ras by promoting GTP/GDP exchange.	bind
25928	5	7072	7	NULL	NULL	0	NULL	statement 3	NULL		activates	NULL				p21ras	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_38_23304_s_139	8798530	2 Recent studies suggest that JNK binds to growth factor receptor binding protein 2 ( 11), the adapter protein that links tyrosine kinase receptors to the SOS protein, which, in turn, activates p21 ras by promoting GTP/GDP exchange.	bind
25929	6	7072	7	10	NULL	0	NULL	statement 5	NULL		occurs by	NULL				GTP/GDP exchange	NULL	promoting			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_38_23304_s_139	8798530	2 Recent studies suggest that JNK binds to growth factor receptor binding protein 2 ( 11), the adapter protein that links tyrosine kinase receptors to the SOS protein, which, in turn, activates p21 ras by promoting GTP/GDP exchange.	bind
22188	1	7073	6	13	NULL	NULL	NULL	gp41	GP		assembles onto					gp32-ssDNA complexes	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_33_20198_s_33	8702746	2 Second, gp59-dependent assembly of gp41 onto gp32-ssDNA complexes, as measured by activation of the helicase's ssDNA-stimulated nucleotidase activity, is inhibited by excess free gp32, suggesting that gp59 must contact ssDNA-bound gp32 molecules in order to promote helicase-ssDNA assembly (Morrical  et al., 1994  ).	bind
22189	2	7073	6	13	NULL	NULL	NULL	statement 1	Process		is dependent on					gp59	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_33_20198_s_33	8702746	2 Second, gp59-dependent assembly of gp41 onto gp32-ssDNA complexes, as measured by activation of the helicase's ssDNA-stimulated nucleotidase activity, is inhibited by excess free gp32, suggesting that gp59 must contact ssDNA-bound gp32 molecules in order to promote helicase-ssDNA assembly (Morrical  et al., 1994  ).	bind
22190	3	7073	6	13	NULL	NULL	NULL	ssDNA	NucleicAcid		stimulates					nucleotidase 	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_33_20198_s_33	8702746	2 Second, gp59-dependent assembly of gp41 onto gp32-ssDNA complexes, as measured by activation of the helicase's ssDNA-stimulated nucleotidase activity, is inhibited by excess free gp32, suggesting that gp59 must contact ssDNA-bound gp32 molecules in order to promote helicase-ssDNA assembly (Morrical  et al., 1994  ).	bind
22191	4	7073	6	13	NULL	NULL	NULL	gp32	GP	excess of	inhibits					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_33_20198_s_33	8702746	2 Second, gp59-dependent assembly of gp41 onto gp32-ssDNA complexes, as measured by activation of the helicase's ssDNA-stimulated nucleotidase activity, is inhibited by excess free gp32, suggesting that gp59 must contact ssDNA-bound gp32 molecules in order to promote helicase-ssDNA assembly (Morrical  et al., 1994  ).	bind
22192	5	7073	6	13	NULL	NULL	NULL	gp59	GP		promote					helicase-ssDNA 	GP	assembly of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_33_20198_s_33	8702746	2 Second, gp59-dependent assembly of gp41 onto gp32-ssDNA complexes, as measured by activation of the helicase's ssDNA-stimulated nucleotidase activity, is inhibited by excess free gp32, suggesting that gp59 must contact ssDNA-bound gp32 molecules in order to promote helicase-ssDNA assembly (Morrical  et al., 1994  ).	bind
22193	6	7073	6	13	NULL	NULL	NULL	gp39	GP		contact		must			statement 8	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_33_20198_s_33	8702746	2 Second, gp59-dependent assembly of gp41 onto gp32-ssDNA complexes, as measured by activation of the helicase's ssDNA-stimulated nucleotidase activity, is inhibited by excess free gp32, suggesting that gp59 must contact ssDNA-bound gp32 molecules in order to promote helicase-ssDNA assembly (Morrical  et al., 1994  ).	bind
22194	7	7073	6	13	NULL	NULL	NULL	statement 5	Process		promote					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_33_20198_s_33	8702746	2 Second, gp59-dependent assembly of gp41 onto gp32-ssDNA complexes, as measured by activation of the helicase's ssDNA-stimulated nucleotidase activity, is inhibited by excess free gp32, suggesting that gp59 must contact ssDNA-bound gp32 molecules in order to promote helicase-ssDNA assembly (Morrical  et al., 1994  ).	bind
46420	8	7073	6	13	NULL	NULL	NULL	ssDNA	NucleicAcid		bind					gp32 molecules	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_33_20198_s_33	8702746	2 Second, gp59-dependent assembly of gp41 onto gp32-ssDNA complexes, as measured by activation of the helicase's ssDNA-stimulated nucleotidase activity, is inhibited by excess free gp32, suggesting that gp59 must contact ssDNA-bound gp32 molecules in order to promote helicase-ssDNA assembly (Morrical  et al., 1994  ).	bind
25930	1	7073	7	NULL	NULL	0	NULL	gp41	NULL		assemble onto	NULL				gp32-ssDNA complex	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_33_20198_s_33	8702746	2 Second, gp59-dependent assembly of gp41 onto gp32-ssDNA complexes, as measured by activation of the helicase's ssDNA-stimulated nucleotidase activity, is inhibited by excess free gp32, suggesting that gp59 must contact ssDNA-bound gp32 molecules in order to promote helicase-ssDNA assembly (Morrical  et al., 1994  ).	bind
25931	2	7073	7	NULL	NULL	0	NULL	statement 1	NULL		depends on	NULL				gp59	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_33_20198_s_33	8702746	2 Second, gp59-dependent assembly of gp41 onto gp32-ssDNA complexes, as measured by activation of the helicase's ssDNA-stimulated nucleotidase activity, is inhibited by excess free gp32, suggesting that gp59 must contact ssDNA-bound gp32 molecules in order to promote helicase-ssDNA assembly (Morrical  et al., 1994  ).	bind
25932	3	7073	7	NULL	NULL	0	NULL	gp32	NULL	excess of	inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_33_20198_s_33	8702746	2 Second, gp59-dependent assembly of gp41 onto gp32-ssDNA complexes, as measured by activation of the helicase's ssDNA-stimulated nucleotidase activity, is inhibited by excess free gp32, suggesting that gp59 must contact ssDNA-bound gp32 molecules in order to promote helicase-ssDNA assembly (Morrical  et al., 1994  ).	bind
25933	4	7073	7	10	NULL	0	NULL	gp59	NULL		contact	NULL	must			statement 8	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_33_20198_s_33	8702746	2 Second, gp59-dependent assembly of gp41 onto gp32-ssDNA complexes, as measured by activation of the helicase's ssDNA-stimulated nucleotidase activity, is inhibited by excess free gp32, suggesting that gp59 must contact ssDNA-bound gp32 molecules in order to promote helicase-ssDNA assembly (Morrical  et al., 1994  ).	bind
25934	5	7073	7	NULL	NULL	0	NULL	statement 3	NULL		suggests	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_33_20198_s_33	8702746	2 Second, gp59-dependent assembly of gp41 onto gp32-ssDNA complexes, as measured by activation of the helicase's ssDNA-stimulated nucleotidase activity, is inhibited by excess free gp32, suggesting that gp59 must contact ssDNA-bound gp32 molecules in order to promote helicase-ssDNA assembly (Morrical  et al., 1994  ).	bind
25935	6	7073	7	NULL	NULL	0	NULL	statement 4	NULL		promote	NULL				helicase-ssDNA 	NULL	assembly of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_33_20198_s_33	8702746	2 Second, gp59-dependent assembly of gp41 onto gp32-ssDNA complexes, as measured by activation of the helicase's ssDNA-stimulated nucleotidase activity, is inhibited by excess free gp32, suggesting that gp59 must contact ssDNA-bound gp32 molecules in order to promote helicase-ssDNA assembly (Morrical  et al., 1994  ).	bind
28025	7	7073	7	NULL	NULL	0	NULL	ssDNA	NULL		stimulates	NULL				nucleotidase	NULL	activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_33_20198_s_33	8702746	2 Second, gp59-dependent assembly of gp41 onto gp32-ssDNA complexes, as measured by activation of the helicase's ssDNA-stimulated nucleotidase activity, is inhibited by excess free gp32, suggesting that gp59 must contact ssDNA-bound gp32 molecules in order to promote helicase-ssDNA assembly (Morrical  et al., 1994  ).	bind
46421	8	7073	7	10	NULL	0	NULL	ssDNA	NULL		bind	NULL				gp32 molecules	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_33_20198_s_33	8702746	2 Second, gp59-dependent assembly of gp41 onto gp32-ssDNA complexes, as measured by activation of the helicase's ssDNA-stimulated nucleotidase activity, is inhibited by excess free gp32, suggesting that gp59 must contact ssDNA-bound gp32 molecules in order to promote helicase-ssDNA assembly (Morrical  et al., 1994  ).	bind
21939	1	7074	6	13	NULL	NULL	NULL	Serine/arginine-rich proteins	GP		is a type of					RNA transactivating factors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_2_910_s_253	9422749	2 Serine/arginine-rich (SR) proteins and pyrimidine tract-binding protein are known RNA transactivating factors that bind to these  cis-elements and affect exon inclusion and 5  splice selection ( 21).	bind
21948	2	7074	6	13	NULL	NULL	NULL	pyrimidine tract-binding protein	GP		is a type of					RNA transactivating factors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_2_910_s_253	9422749	2 Serine/arginine-rich (SR) proteins and pyrimidine tract-binding protein are known RNA transactivating factors that bind to these  cis-elements and affect exon inclusion and 5  splice selection ( 21).	bind
21949	3	7074	6	13	NULL	NULL	NULL	Serine/arginine-rich proteins	GP		is 					SR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_2_910_s_253	9422749	2 Serine/arginine-rich (SR) proteins and pyrimidine tract-binding protein are known RNA transactivating factors that bind to these  cis-elements and affect exon inclusion and 5  splice selection ( 21).	bind
21950	4	7074	6	13	NULL	NULL	NULL	statement 1	GP		bind									cis-elements	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_2_910_s_253	9422749	2 Serine/arginine-rich (SR) proteins and pyrimidine tract-binding protein are known RNA transactivating factors that bind to these  cis-elements and affect exon inclusion and 5  splice selection ( 21).	bind
21951	5	7074	6	13	NULL	NULL	NULL	statement 4	Process		affect					exon inclusion	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_2_910_s_253	9422749	2 Serine/arginine-rich (SR) proteins and pyrimidine tract-binding protein are known RNA transactivating factors that bind to these  cis-elements and affect exon inclusion and 5  splice selection ( 21).	bind
21952	6	7074	6	13	NULL	NULL	NULL	statement 4	Process		affect					splice selection	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_2_910_s_253	9422749	2 Serine/arginine-rich (SR) proteins and pyrimidine tract-binding protein are known RNA transactivating factors that bind to these  cis-elements and affect exon inclusion and 5  splice selection ( 21).	bind
21953	7	7074	6	13	NULL	NULL	NULL	statement 2	GP		bind									cis-elements	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_2_910_s_253	9422749	2 Serine/arginine-rich (SR) proteins and pyrimidine tract-binding protein are known RNA transactivating factors that bind to these  cis-elements and affect exon inclusion and 5  splice selection ( 21).	bind
21954	8	7074	6	13	NULL	NULL	NULL	statement 7	Process		affect					exon inclusion	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_2_910_s_253	9422749	2 Serine/arginine-rich (SR) proteins and pyrimidine tract-binding protein are known RNA transactivating factors that bind to these  cis-elements and affect exon inclusion and 5  splice selection ( 21).	bind
21955	9	7074	6	13	NULL	NULL	NULL	statement 7	Process		affect					splice selection	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_2_910_s_253	9422749	2 Serine/arginine-rich (SR) proteins and pyrimidine tract-binding protein are known RNA transactivating factors that bind to these  cis-elements and affect exon inclusion and 5  splice selection ( 21).	bind
25936	1	7074	7	NULL	NULL	0	NULL	SR protein	NULL		is a type of	NULL				RNA transactivating factors	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_2_910_s_253	9422749	2 Serine/arginine-rich (SR) proteins and pyrimidine tract-binding protein are known RNA transactivating factors that bind to these  cis-elements and affect exon inclusion and 5  splice selection ( 21).	bind
25937	2	7074	7	NULL	NULL	0	NULL	pyrimidine tract-binding protein	NULL		is a type of	NULL				RNA transactivating factors	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_2_910_s_253	9422749	2 Serine/arginine-rich (SR) proteins and pyrimidine tract-binding protein are known RNA transactivating factors that bind to these  cis-elements and affect exon inclusion and 5  splice selection ( 21).	bind
25938	3	7074	7	NULL	NULL	0	NULL	SR protein	NULL		bind	NULL					NULL			cis-elements	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_2_910_s_253	9422749	2 Serine/arginine-rich (SR) proteins and pyrimidine tract-binding protein are known RNA transactivating factors that bind to these  cis-elements and affect exon inclusion and 5  splice selection ( 21).	bind
25939	4	7074	7	NULL	NULL	0	NULL	pyrimidine tract-binding protein	NULL		bind	NULL					NULL			cis-elements	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_2_910_s_253	9422749	2 Serine/arginine-rich (SR) proteins and pyrimidine tract-binding protein are known RNA transactivating factors that bind to these  cis-elements and affect exon inclusion and 5  splice selection ( 21).	bind
25940	5	7074	7	NULL	NULL	0	NULL	statement 3	NULL		affect	NULL				exon inclusion	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_2_910_s_253	9422749	2 Serine/arginine-rich (SR) proteins and pyrimidine tract-binding protein are known RNA transactivating factors that bind to these  cis-elements and affect exon inclusion and 5  splice selection ( 21).	bind
25941	6	7074	7	NULL	NULL	0	NULL	statement 3	NULL		affect	NULL				splice selection 	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_2_910_s_253	9422749	2 Serine/arginine-rich (SR) proteins and pyrimidine tract-binding protein are known RNA transactivating factors that bind to these  cis-elements and affect exon inclusion and 5  splice selection ( 21).	bind
25942	7	7074	7	NULL	NULL	0	NULL	statement 4	NULL		affect	NULL				exon inclusion	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_2_910_s_253	9422749	2 Serine/arginine-rich (SR) proteins and pyrimidine tract-binding protein are known RNA transactivating factors that bind to these  cis-elements and affect exon inclusion and 5  splice selection ( 21).	bind
25943	8	7074	7	NULL	NULL	0	NULL	statement 4	NULL		affect	NULL				splice selection	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_2_910_s_253	9422749	2 Serine/arginine-rich (SR) proteins and pyrimidine tract-binding protein are known RNA transactivating factors that bind to these  cis-elements and affect exon inclusion and 5  splice selection ( 21).	bind
22195	1	7075	6	13	NULL	NULL	NULL	rGPBP	GP		bind					protein	GP	human;;recombinant	alpha1 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40392_s_265	11007769	2 Similar pattern to that shown in Fig.  3 D was obtained when assessing the binding of rGPBP or rGPBPdelta26 to recombinant proteins representing the human highly homologous alpha1 and alpha5(IV)NC1 domains; however, no significant material bound to the recombinant material representing the alpha2-, alpha4 , and alpha6(IV)NC1 counterparts.	bind
22196	2	7075	6	13	NULL	NULL	NULL	rGPBP	GP		bind			delta26		protein	GP	human;;recombinant	alpha1 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40392_s_265	11007769	2 Similar pattern to that shown in Fig.  3 D was obtained when assessing the binding of rGPBP or rGPBPdelta26 to recombinant proteins representing the human highly homologous alpha1 and alpha5(IV)NC1 domains; however, no significant material bound to the recombinant material representing the alpha2-, alpha4 , and alpha6(IV)NC1 counterparts.	bind
22197	3	7075	6	13	NULL	NULL	NULL	rGPBP	GP		bind					protein	GP	human;;recombinant	alpha5(IV)NC1 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40392_s_265	11007769	2 Similar pattern to that shown in Fig.  3 D was obtained when assessing the binding of rGPBP or rGPBPdelta26 to recombinant proteins representing the human highly homologous alpha1 and alpha5(IV)NC1 domains; however, no significant material bound to the recombinant material representing the alpha2-, alpha4 , and alpha6(IV)NC1 counterparts.	bind
22198	4	7075	6	13	NULL	NULL	NULL	rGPBP	GP		bind			delta26		protein	GP	human;;recombinant	alpha5(IV)NC1 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40392_s_265	11007769	2 Similar pattern to that shown in Fig.  3 D was obtained when assessing the binding of rGPBP or rGPBPdelta26 to recombinant proteins representing the human highly homologous alpha1 and alpha5(IV)NC1 domains; however, no significant material bound to the recombinant material representing the alpha2-, alpha4 , and alpha6(IV)NC1 counterparts.	bind
22199	5	7075	6	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40392_s_265	11007769	2 Similar pattern to that shown in Fig.  3 D was obtained when assessing the binding of rGPBP or rGPBPdelta26 to recombinant proteins representing the human highly homologous alpha1 and alpha5(IV)NC1 domains; however, no significant material bound to the recombinant material representing the alpha2-, alpha4 , and alpha6(IV)NC1 counterparts.	bind
22200	6	7075	6	13	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40392_s_265	11007769	2 Similar pattern to that shown in Fig.  3 D was obtained when assessing the binding of rGPBP or rGPBPdelta26 to recombinant proteins representing the human highly homologous alpha1 and alpha5(IV)NC1 domains; however, no significant material bound to the recombinant material representing the alpha2-, alpha4 , and alpha6(IV)NC1 counterparts.	bind
22201	7	7075	6	13	NULL	NULL	NULL	rGPBP	GP		does not bind					protein	GP	human;;recombinant	alpha2 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40392_s_265	11007769	2 Similar pattern to that shown in Fig.  3 D was obtained when assessing the binding of rGPBP or rGPBPdelta26 to recombinant proteins representing the human highly homologous alpha1 and alpha5(IV)NC1 domains; however, no significant material bound to the recombinant material representing the alpha2-, alpha4 , and alpha6(IV)NC1 counterparts.	bind
22202	8	7075	6	13	NULL	NULL	NULL	rGPBP	GP		does not bind					protein	GP	human;;recombinant	alpha4 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40392_s_265	11007769	2 Similar pattern to that shown in Fig.  3 D was obtained when assessing the binding of rGPBP or rGPBPdelta26 to recombinant proteins representing the human highly homologous alpha1 and alpha5(IV)NC1 domains; however, no significant material bound to the recombinant material representing the alpha2-, alpha4 , and alpha6(IV)NC1 counterparts.	bind
22203	9	7075	6	13	NULL	NULL	NULL	rGPBP	GP		does not bind					protein	GP	human;;recombinant	alpha6(IV)NC1 		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40392_s_265	11007769	2 Similar pattern to that shown in Fig.  3 D was obtained when assessing the binding of rGPBP or rGPBPdelta26 to recombinant proteins representing the human highly homologous alpha1 and alpha5(IV)NC1 domains; however, no significant material bound to the recombinant material representing the alpha2-, alpha4 , and alpha6(IV)NC1 counterparts.	bind
22204	10	7075	6	13	NULL	NULL	NULL	rGPBP	GP		does not bind			delta26		protein	GP	human;;recombinant	alpha2 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40392_s_265	11007769	2 Similar pattern to that shown in Fig.  3 D was obtained when assessing the binding of rGPBP or rGPBPdelta26 to recombinant proteins representing the human highly homologous alpha1 and alpha5(IV)NC1 domains; however, no significant material bound to the recombinant material representing the alpha2-, alpha4 , and alpha6(IV)NC1 counterparts.	bind
22205	11	7075	6	13	NULL	NULL	NULL	rGPBP	GP		does not bind			delta26		protein	GP	human;;recombinant	alpha4 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40392_s_265	11007769	2 Similar pattern to that shown in Fig.  3 D was obtained when assessing the binding of rGPBP or rGPBPdelta26 to recombinant proteins representing the human highly homologous alpha1 and alpha5(IV)NC1 domains; however, no significant material bound to the recombinant material representing the alpha2-, alpha4 , and alpha6(IV)NC1 counterparts.	bind
22206	12	7075	6	13	NULL	NULL	NULL	rGPBP	GP		does not bind			delta26		protein	GP	human;;recombinant	alpha6(IV)NC1		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40392_s_265	11007769	2 Similar pattern to that shown in Fig.  3 D was obtained when assessing the binding of rGPBP or rGPBPdelta26 to recombinant proteins representing the human highly homologous alpha1 and alpha5(IV)NC1 domains; however, no significant material bound to the recombinant material representing the alpha2-, alpha4 , and alpha6(IV)NC1 counterparts.	bind
25946	1	7075	7	10	NULL	0	NULL	rGPBP	NULL		bind	NULL				proteins	NULL	human;;highly homologous;;recombinant	alpha1 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40392_s_265	11007769	2 Similar pattern to that shown in Fig.  3 D was obtained when assessing the binding of rGPBP or rGPBPdelta26 to recombinant proteins representing the human highly homologous alpha1 and alpha5(IV)NC1 domains; however, no significant material bound to the recombinant material representing the alpha2-, alpha4 , and alpha6(IV)NC1 counterparts.	bind
25947	2	7075	7	10	NULL	0	NULL	rGPBP	NULL		bind	NULL				proteins	NULL	human;;highly homologous;;recombinant	alpha5(IV)NC1 domains		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40392_s_265	11007769	2 Similar pattern to that shown in Fig.  3 D was obtained when assessing the binding of rGPBP or rGPBPdelta26 to recombinant proteins representing the human highly homologous alpha1 and alpha5(IV)NC1 domains; however, no significant material bound to the recombinant material representing the alpha2-, alpha4 , and alpha6(IV)NC1 counterparts.	bind
28472	3	7075	7	10	NULL	0	NULL	 rGPBP	NULL		bind	NULL		delta26		proteins	NULL	human;;highly homologous;;recombinant	alpha1 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40392_s_265	11007769	2 Similar pattern to that shown in Fig.  3 D was obtained when assessing the binding of rGPBP or rGPBPdelta26 to recombinant proteins representing the human highly homologous alpha1 and alpha5(IV)NC1 domains; however, no significant material bound to the recombinant material representing the alpha2-, alpha4 , and alpha6(IV)NC1 counterparts.	bind
28473	4	7075	7	10	NULL	0	NULL	 rGPBP	NULL		bind	NULL		delta26		proteins	NULL	human;;highly homologous;;recombinant	alpha5(IV)NC1 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40392_s_265	11007769	2 Similar pattern to that shown in Fig.  3 D was obtained when assessing the binding of rGPBP or rGPBPdelta26 to recombinant proteins representing the human highly homologous alpha1 and alpha5(IV)NC1 domains; however, no significant material bound to the recombinant material representing the alpha2-, alpha4 , and alpha6(IV)NC1 counterparts.	bind
28474	5	7075	7	10	NULL	0	NULL	rGPBP	NULL		does not bind	NULL				protein	NULL	human;;recombinant	alpha2 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40392_s_265	11007769	2 Similar pattern to that shown in Fig.  3 D was obtained when assessing the binding of rGPBP or rGPBPdelta26 to recombinant proteins representing the human highly homologous alpha1 and alpha5(IV)NC1 domains; however, no significant material bound to the recombinant material representing the alpha2-, alpha4 , and alpha6(IV)NC1 counterparts.	bind
28475	6	7075	7	10	NULL	0	NULL	rGPBP	NULL		does not bind	NULL				protein	NULL	human;;recombinant	alpha4 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40392_s_265	11007769	2 Similar pattern to that shown in Fig.  3 D was obtained when assessing the binding of rGPBP or rGPBPdelta26 to recombinant proteins representing the human highly homologous alpha1 and alpha5(IV)NC1 domains; however, no significant material bound to the recombinant material representing the alpha2-, alpha4 , and alpha6(IV)NC1 counterparts.	bind
28476	7	7075	7	10	NULL	0	NULL	rGPBP	NULL		does not bind	NULL				protein	NULL	human;;recombinant	alpha6(IV)NC1 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40392_s_265	11007769	2 Similar pattern to that shown in Fig.  3 D was obtained when assessing the binding of rGPBP or rGPBPdelta26 to recombinant proteins representing the human highly homologous alpha1 and alpha5(IV)NC1 domains; however, no significant material bound to the recombinant material representing the alpha2-, alpha4 , and alpha6(IV)NC1 counterparts.	bind
30063	8	7075	7	10	NULL	0	NULL	 rGPBP	NULL		does not bind	NULL		delta26		protein	NULL	human;;recombinant	alpha2 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40392_s_265	11007769	2 Similar pattern to that shown in Fig.  3 D was obtained when assessing the binding of rGPBP or rGPBPdelta26 to recombinant proteins representing the human highly homologous alpha1 and alpha5(IV)NC1 domains; however, no significant material bound to the recombinant material representing the alpha2-, alpha4 , and alpha6(IV)NC1 counterparts.	bind
30064	9	7075	7	10	NULL	0	NULL	rGPBP	NULL		does not bind	NULL		delta26		protein	NULL	human;;recombinant	alpha4 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40392_s_265	11007769	2 Similar pattern to that shown in Fig.  3 D was obtained when assessing the binding of rGPBP or rGPBPdelta26 to recombinant proteins representing the human highly homologous alpha1 and alpha5(IV)NC1 domains; however, no significant material bound to the recombinant material representing the alpha2-, alpha4 , and alpha6(IV)NC1 counterparts.	bind
30065	10	7075	7	10	NULL	0	NULL	rGPBP	NULL		does not bind	NULL		delta26		protein	NULL	human;;recombinant	alpha6(IV)NC1 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40392_s_265	11007769	2 Similar pattern to that shown in Fig.  3 D was obtained when assessing the binding of rGPBP or rGPBPdelta26 to recombinant proteins representing the human highly homologous alpha1 and alpha5(IV)NC1 domains; however, no significant material bound to the recombinant material representing the alpha2-, alpha4 , and alpha6(IV)NC1 counterparts.	bind
21956	1	7076	6	13	NULL	NULL	NULL	SF-1	GP		interacts with					p300	GP		amino terminal region		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_8_4585_s_189	9468515	2 Similar to other nuclear receptors, SF-1 interacts with the amino-terminal region of p300; however, SF-1 also binds p300 at the carboxyl-terminal region, which have been shown to interact with several transcription factors including SRC-1 ( 50).	bind
21957	2	7076	6	13	NULL	NULL	NULL	SF-1	GP		bind					p300	GP		carboxyl-terminal region		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_8_4585_s_189	9468515	2 Similar to other nuclear receptors, SF-1 interacts with the amino-terminal region of p300; however, SF-1 also binds p300 at the carboxyl-terminal region, which have been shown to interact with several transcription factors including SRC-1 ( 50).	bind
21958	3	7076	6	13	NULL	NULL	NULL	p300	GP		interact with			carboxyl-terminal region		SRC-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_8_4585_s_189	9468515	2 Similar to other nuclear receptors, SF-1 interacts with the amino-terminal region of p300; however, SF-1 also binds p300 at the carboxyl-terminal region, which have been shown to interact with several transcription factors including SRC-1 ( 50).	bind
27029	4	7076	6	13	NULL	NULL	NULL	SRC-1	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_8_4585_s_189	9468515	2 Similar to other nuclear receptors, SF-1 interacts with the amino-terminal region of p300; however, SF-1 also binds p300 at the carboxyl-terminal region, which have been shown to interact with several transcription factors including SRC-1 ( 50).	bind
25948	1	7076	7	NULL	NULL	0	NULL	SF-1 	NULL		interacts with	NULL				p300	NULL		 amino-terminal		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_8_4585_s_189	9468515	2 Similar to other nuclear receptors, SF-1 interacts with the amino-terminal region of p300; however, SF-1 also binds p300 at the carboxyl-terminal region, which have been shown to interact with several transcription factors including SRC-1 ( 50).	bind
25949	2	7076	7	10	NULL	0	NULL	 SF-1	NULL		bind	NULL				p300	NULL		carboxyl-terminal region		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_8_4585_s_189	9468515	2 Similar to other nuclear receptors, SF-1 interacts with the amino-terminal region of p300; however, SF-1 also binds p300 at the carboxyl-terminal region, which have been shown to interact with several transcription factors including SRC-1 ( 50).	bind
25950	3	7076	7	NULL	NULL	0	NULL	p300	NULL		interacts with	NULL		carboxyl-terminal region		SRC-1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_8_4585_s_189	9468515	2 Similar to other nuclear receptors, SF-1 interacts with the amino-terminal region of p300; however, SF-1 also binds p300 at the carboxyl-terminal region, which have been shown to interact with several transcription factors including SRC-1 ( 50).	bind
28477	4	7076	7	NULL	NULL	0	NULL	SRC-1	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_8_4585_s_189	9468515	2 Similar to other nuclear receptors, SF-1 interacts with the amino-terminal region of p300; however, SF-1 also binds p300 at the carboxyl-terminal region, which have been shown to interact with several transcription factors including SRC-1 ( 50).	bind
21959	1	7077	6	13	NULL	NULL	NULL	SEMA3A/Sema3A	GP		bind					neuropilin-1 receptor	GP	endothelial			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39647_s_227	10993894	2 Similarly, binding of the well known guidance signal SEMA3A/Sema3A to the endothelial neuropilin-1 receptor, which mediates repulsive signals, also leads to a reduced cell motility ( 41).	bind
21960	2	7077	6	13	NULL	NULL	NULL	statement 1	Process		mediates					repulsive signals	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39647_s_227	10993894	2 Similarly, binding of the well known guidance signal SEMA3A/Sema3A to the endothelial neuropilin-1 receptor, which mediates repulsive signals, also leads to a reduced cell motility ( 41).	bind
21961	3	7077	6	13	NULL	NULL	NULL	statement 1	Process		leads to					cell motility	Process	reduced			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39647_s_227	10993894	2 Similarly, binding of the well known guidance signal SEMA3A/Sema3A to the endothelial neuropilin-1 receptor, which mediates repulsive signals, also leads to a reduced cell motility ( 41).	bind
25951	1	7077	7	NULL	NULL	0	NULL	 SEMA3A/Sema3A 	NULL		binds to	NULL				neuropilin-1 receptor	NULL	endothelial			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_50_39647_s_227	10993894	2 Similarly, binding of the well known guidance signal SEMA3A/Sema3A to the endothelial neuropilin-1 receptor, which mediates repulsive signals, also leads to a reduced cell motility ( 41).	bind
25952	2	7077	7	NULL	NULL	0	NULL	statement 1	NULL		mediates	NULL				repulsive signals	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_50_39647_s_227	10993894	2 Similarly, binding of the well known guidance signal SEMA3A/Sema3A to the endothelial neuropilin-1 receptor, which mediates repulsive signals, also leads to a reduced cell motility ( 41).	bind
25953	3	7077	7	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				cell motility	NULL	reduced			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_50_39647_s_227	10993894	2 Similarly, binding of the well known guidance signal SEMA3A/Sema3A to the endothelial neuropilin-1 receptor, which mediates repulsive signals, also leads to a reduced cell motility ( 41).	bind
21962	1	7078	6	13	NULL	NULL	NULL	aminopeptidases	GP	Manduca sexta	bind					Cry1A toxins	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_16_13863_s_16	11836242	2 Similarly, in  Manduca sexta and  Bombyx mori, aminopeptidases and the cadherin-like proteins bind Cry1A toxins as well ( 10-14).	bind
21963	2	7078	6	13	NULL	NULL	NULL	aminopeptidases	GP	bombyx mori	bind					Cry1A toxins	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_16_13863_s_16	11836242	2 Similarly, in  Manduca sexta and  Bombyx mori, aminopeptidases and the cadherin-like proteins bind Cry1A toxins as well ( 10-14).	bind
21964	3	7078	6	13	NULL	NULL	NULL	cadherin-like proteins	GP	Manduca sexta	bind					Cry1A toxins	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_16_13863_s_16	11836242	2 Similarly, in  Manduca sexta and  Bombyx mori, aminopeptidases and the cadherin-like proteins bind Cry1A toxins as well ( 10-14).	bind
21965	4	7078	6	13	NULL	NULL	NULL	cadherin-like proteins	GP	bombyx mori	bind					Cry1A toxins	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_16_13863_s_16	11836242	2 Similarly, in  Manduca sexta and  Bombyx mori, aminopeptidases and the cadherin-like proteins bind Cry1A toxins as well ( 10-14).	bind
25954	1	7078	7	NULL	NULL	0	NULL	aminopeptidases	NULL	Manduca sexta 	bind	NULL				Cry1A toxins	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_16_13863_s_16	11836242	2 Similarly, in  Manduca sexta and  Bombyx mori, aminopeptidases and the cadherin-like proteins bind Cry1A toxins as well ( 10-14).	bind
25955	2	7078	7	NULL	NULL	0	NULL	aminopeptidases 	NULL	Bombyx mori	bind	NULL				Cry1A toxins	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_16_13863_s_16	11836242	2 Similarly, in  Manduca sexta and  Bombyx mori, aminopeptidases and the cadherin-like proteins bind Cry1A toxins as well ( 10-14).	bind
25956	3	7078	7	NULL	NULL	0	NULL	cadherin-like proteins	NULL	Manduca sexta	bind	NULL				Cry1A toxins	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_16_13863_s_16	11836242	2 Similarly, in  Manduca sexta and  Bombyx mori, aminopeptidases and the cadherin-like proteins bind Cry1A toxins as well ( 10-14).	bind
25957	4	7078	7	NULL	NULL	0	NULL	 cadherin-like proteins	NULL	Bombyx mori	bind	NULL				Cry1A toxins	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_16_13863_s_16	11836242	2 Similarly, in  Manduca sexta and  Bombyx mori, aminopeptidases and the cadherin-like proteins bind Cry1A toxins as well ( 10-14).	bind
21966	1	7079	6	13	NULL	NULL	NULL	syndecan-4	GP		bind					PIP2	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_17_10624_s_34	9553124	2 Since syndecan-4 can bind PIP2 and activate PKC, we investigated whether PIP2 and syndecan-4 act synergistically to activate PKC, representing an alternative pathway to those previously described.	bind
21967	2	7079	6	13	NULL	NULL	NULL	statement 1	Process		activate					PKC	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_17_10624_s_34	9553124	2 Since syndecan-4 can bind PIP2 and activate PKC, we investigated whether PIP2 and syndecan-4 act synergistically to activate PKC, representing an alternative pathway to those previously described.	bind
25958	1	7079	7	NULL	NULL	0	NULL	syndecan-4	NULL		bind	NULL				 PIP2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_17_10624_s_34	9553124	2 Since syndecan-4 can bind PIP2 and activate PKC, we investigated whether PIP2 and syndecan-4 act synergistically to activate PKC, representing an alternative pathway to those previously described.	bind
25959	2	7079	7	NULL	NULL	0	NULL	statement 1	NULL		activate	NULL				PKC	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_17_10624_s_34	9553124	2 Since syndecan-4 can bind PIP2 and activate PKC, we investigated whether PIP2 and syndecan-4 act synergistically to activate PKC, representing an alternative pathway to those previously described.	bind
21968	1	7080	6	13	NULL	NULL	NULL	His6-sCD4	GP		bind					PDP-CB1	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_508_1_67_s_24	11707270	2 specifically displaced the binding of His6-sCD4 to PDPs CB1 and CB8, indicating that anti-CD4 PDPs recognize an epitope on the CD4 molecule closely related or similar to that identified for the 13B8.	bind
21969	2	7080	6	13	NULL	NULL	NULL	His6-sCD4	GP		bind					PDP-CB8	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_508_1_67_s_24	11707270	2 specifically displaced the binding of His6-sCD4 to PDPs CB1 and CB8, indicating that anti-CD4 PDPs recognize an epitope on the CD4 molecule closely related or similar to that identified for the 13B8.	bind
21970	3	7080	6	13	NULL	NULL	NULL	anti-CD4 PDP	GP		recognize					CD4 molecule epitope	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_508_1_67_s_24	11707270	2 specifically displaced the binding of His6-sCD4 to PDPs CB1 and CB8, indicating that anti-CD4 PDPs recognize an epitope on the CD4 molecule closely related or similar to that identified for the 13B8.	bind
25973	1	7080	7	NULL	NULL	0	NULL	His6-sCD4	NULL		bind	NULL				PDPs CB1 	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_508_1_67_s_24	11707270	2 specifically displaced the binding of His6-sCD4 to PDPs CB1 and CB8, indicating that anti-CD4 PDPs recognize an epitope on the CD4 molecule closely related or similar to that identified for the 13B8.	bind
25975	2	7080	7	NULL	NULL	0	NULL	His6-sCD4 	NULL		bind	NULL				PDPs CB8	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_508_1_67_s_24	11707270	2 specifically displaced the binding of His6-sCD4 to PDPs CB1 and CB8, indicating that anti-CD4 PDPs recognize an epitope on the CD4 molecule closely related or similar to that identified for the 13B8.	bind
25977	3	7080	7	NULL	NULL	0	NULL	anti-CD4 PDPs	NULL		recognize	NULL				CD4 molecule epitope	NULL				NULL		NULL	NULL	NULL	NULL	gw60_febslett_508_1_67_s_24	11707270	2 specifically displaced the binding of His6-sCD4 to PDPs CB1 and CB8, indicating that anti-CD4 PDPs recognize an epitope on the CD4 molecule closely related or similar to that identified for the 13B8.	bind
25978	4	7080	7	NULL	NULL	0	NULL	CD4 molecule epitope	NULL		is similar to	NULL				13B8	NULL	identified for			NULL		NULL	NULL	NULL	NULL	gw60_febslett_508_1_67_s_24	11707270	2 specifically displaced the binding of His6-sCD4 to PDPs CB1 and CB8, indicating that anti-CD4 PDPs recognize an epitope on the CD4 molecule closely related or similar to that identified for the 13B8.	bind
21971	1	7082	6	13	NULL	NULL	NULL	ProX	GP		bind		high affinity;;specificity			GB	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_46_48270_s_42	15308642	2 Substrate binding assays with radiolabeled glycine betaine and competition experiments with other compatible solutes revealed that ProX binds both GB and PB with high affinity and specificity at room temperature with an apparent  KD of 60 and 50 nM, respectively.	bind
21972	2	7082	6	13	NULL	NULL	NULL	ProX	GP		bind		high affinity;; specificity			PB	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_46_48270_s_42	15308642	2 Substrate binding assays with radiolabeled glycine betaine and competition experiments with other compatible solutes revealed that ProX binds both GB and PB with high affinity and specificity at room temperature with an apparent  KD of 60 and 50 nM, respectively.	bind
25987	1	7082	7	NULL	NULL	0	NULL	ProX	NULL		binds	NULL	high affinity;;specificity			GB	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_46_48270_s_42	15308642	2 Substrate binding assays with radiolabeled glycine betaine and competition experiments with other compatible solutes revealed that ProX binds both GB and PB with high affinity and specificity at room temperature with an apparent  KD of 60 and 50 nM, respectively.	bind
25988	2	7082	7	NULL	NULL	0	NULL	Prox	NULL		binds	NULL	high affinity;;specificity			PB	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_46_48270_s_42	15308642	2 Substrate binding assays with radiolabeled glycine betaine and competition experiments with other compatible solutes revealed that ProX binds both GB and PB with high affinity and specificity at room temperature with an apparent  KD of 60 and 50 nM, respectively.	bind
21973	1	7083	6	13	NULL	NULL	NULL	Rad3 protein	GP		bind		directly			SSL2/Rad25	GP				NULL	yeast	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_43_33260_s_211	10924514	2 Such interactions have also been reported in the yeast in which Rad3 protein binds directly to both SSL2/Rad25 and SSL1 proteins ( 33).	bind
21974	2	7083	6	13	NULL	NULL	NULL	Rad3 protein	GP		bind		directly			SSL1 protein	GP				NULL	yeast	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_43_33260_s_211	10924514	2 Such interactions have also been reported in the yeast in which Rad3 protein binds directly to both SSL2/Rad25 and SSL1 proteins ( 33).	bind
25990	1	7083	7	NULL	NULL	0	NULL	Rad3 protein	NULL		binds	NULL	directly			SSL2/Rad25	NULL				NULL	yeast	0	NULL	NULL	NULL	gw60_jbiolchem_275_43_33260_s_211	10924514	2 Such interactions have also been reported in the yeast in which Rad3 protein binds directly to both SSL2/Rad25 and SSL1 proteins ( 33).	bind
25992	2	7083	7	NULL	NULL	0	NULL	Rad3 protein	NULL		binds	NULL	directly			SSL1 proteins	NULL				NULL	yeast	0	NULL	NULL	NULL	gw60_jbiolchem_275_43_33260_s_211	10924514	2 Such interactions have also been reported in the yeast in which Rad3 protein binds directly to both SSL2/Rad25 and SSL1 proteins ( 33).	bind
22207	1	7084	6	13	NULL	NULL	NULL	SV-150	GP		is composed of								amino acids 150-186		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_42_27182_s_169	9765238	2 SV-150, composed of amino acids 150-186, is an elongated version of the biologically inactive SV-163 peptide ( 32) that inhibits virus-mediated erythrocyte hemolysis at doses ~50% that of SV-473.2 SV-269 is a leucine zipper motif which specifically binds Sendai virions and inhibits virus-mediated hemolysis ( 43).	bind
22208	2	7084	6	13	NULL	NULL	NULL	SV150	GP		is an elongated version of					SV163 peptide	GP	biologically inactive			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_42_27182_s_169	9765238	2 SV-150, composed of amino acids 150-186, is an elongated version of the biologically inactive SV-163 peptide ( 32) that inhibits virus-mediated erythrocyte hemolysis at doses ~50% that of SV-473.2 SV-269 is a leucine zipper motif which specifically binds Sendai virions and inhibits virus-mediated hemolysis ( 43).	bind
22209	3	7084	6	13	NULL	NULL	NULL	SV-163 peptide	GP		inhibits					erythrocyte hemolysis	MedicalFinding	virus mediated			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_42_27182_s_169	9765238	2 SV-150, composed of amino acids 150-186, is an elongated version of the biologically inactive SV-163 peptide ( 32) that inhibits virus-mediated erythrocyte hemolysis at doses ~50% that of SV-473.2 SV-269 is a leucine zipper motif which specifically binds Sendai virions and inhibits virus-mediated hemolysis ( 43).	bind
22210	4	7084	6	13	NULL	NULL	NULL	SV-269	GP		is a type of					leucine zipper motif	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_42_27182_s_169	9765238	2 SV-150, composed of amino acids 150-186, is an elongated version of the biologically inactive SV-163 peptide ( 32) that inhibits virus-mediated erythrocyte hemolysis at doses ~50% that of SV-473.2 SV-269 is a leucine zipper motif which specifically binds Sendai virions and inhibits virus-mediated hemolysis ( 43).	bind
22211	5	7084	6	13	NULL	NULL	NULL	statement 4	GP		bind		specifically			Sendai virions	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_42_27182_s_169	9765238	2 SV-150, composed of amino acids 150-186, is an elongated version of the biologically inactive SV-163 peptide ( 32) that inhibits virus-mediated erythrocyte hemolysis at doses ~50% that of SV-473.2 SV-269 is a leucine zipper motif which specifically binds Sendai virions and inhibits virus-mediated hemolysis ( 43).	bind
22212	6	7084	6	13	NULL	NULL	NULL	statement 4	Process		inhibits					hemolysis	MedicalFinding	virus mediated			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_42_27182_s_169	9765238	2 SV-150, composed of amino acids 150-186, is an elongated version of the biologically inactive SV-163 peptide ( 32) that inhibits virus-mediated erythrocyte hemolysis at doses ~50% that of SV-473.2 SV-269 is a leucine zipper motif which specifically binds Sendai virions and inhibits virus-mediated hemolysis ( 43).	bind
25994	1	7084	7	10	NULL	0	NULL	SV-150	NULL		is composed of	NULL					NULL		amino acids 150-186		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_42_27182_s_169	9765238	2 SV-150, composed of amino acids 150-186, is an elongated version of the biologically inactive SV-163 peptide ( 32) that inhibits virus-mediated erythrocyte hemolysis at doses ~50% that of SV-473.2 SV-269 is a leucine zipper motif which specifically binds Sendai virions and inhibits virus-mediated hemolysis ( 43).	bind
25995	2	7084	7	NULL	NULL	0	NULL	SV-150	NULL		is an elongated version of	NULL				SV-163 peptide	NULL	biologically inactive			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_42_27182_s_169	9765238	2 SV-150, composed of amino acids 150-186, is an elongated version of the biologically inactive SV-163 peptide ( 32) that inhibits virus-mediated erythrocyte hemolysis at doses ~50% that of SV-473.2 SV-269 is a leucine zipper motif which specifically binds Sendai virions and inhibits virus-mediated hemolysis ( 43).	bind
25996	3	7084	7	NULL	NULL	0	NULL	virus	NULL		mediates	NULL				erythrocyte hemolysis 	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_42_27182_s_169	9765238	2 SV-150, composed of amino acids 150-186, is an elongated version of the biologically inactive SV-163 peptide ( 32) that inhibits virus-mediated erythrocyte hemolysis at doses ~50% that of SV-473.2 SV-269 is a leucine zipper motif which specifically binds Sendai virions and inhibits virus-mediated hemolysis ( 43).	bind
25997	4	7084	7	NULL	NULL	0	NULL	SV-150	NULL		inhibits	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_42_27182_s_169	9765238	2 SV-150, composed of amino acids 150-186, is an elongated version of the biologically inactive SV-163 peptide ( 32) that inhibits virus-mediated erythrocyte hemolysis at doses ~50% that of SV-473.2 SV-269 is a leucine zipper motif which specifically binds Sendai virions and inhibits virus-mediated hemolysis ( 43).	bind
25998	5	7084	7	NULL	NULL	0	NULL	SV-473	NULL		inhibits	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_42_27182_s_169	9765238	2 SV-150, composed of amino acids 150-186, is an elongated version of the biologically inactive SV-163 peptide ( 32) that inhibits virus-mediated erythrocyte hemolysis at doses ~50% that of SV-473.2 SV-269 is a leucine zipper motif which specifically binds Sendai virions and inhibits virus-mediated hemolysis ( 43).	bind
25999	6	7084	7	NULL	NULL	0	NULL	statement 4	NULL	efficiency of	is greater than	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_42_27182_s_169	9765238	2 SV-150, composed of amino acids 150-186, is an elongated version of the biologically inactive SV-163 peptide ( 32) that inhibits virus-mediated erythrocyte hemolysis at doses ~50% that of SV-473.2 SV-269 is a leucine zipper motif which specifically binds Sendai virions and inhibits virus-mediated hemolysis ( 43).	bind
26000	7	7084	7	10	NULL	0	NULL	SV-269	NULL		is a type of	NULL				leucine zipper motif	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_42_27182_s_169	9765238	2 SV-150, composed of amino acids 150-186, is an elongated version of the biologically inactive SV-163 peptide ( 32) that inhibits virus-mediated erythrocyte hemolysis at doses ~50% that of SV-473.2 SV-269 is a leucine zipper motif which specifically binds Sendai virions and inhibits virus-mediated hemolysis ( 43).	bind
26001	8	7084	7	10	NULL	0	NULL	statement 7	NULL		binds	NULL	specifically			Sendai virions	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_42_27182_s_169	9765238	2 SV-150, composed of amino acids 150-186, is an elongated version of the biologically inactive SV-163 peptide ( 32) that inhibits virus-mediated erythrocyte hemolysis at doses ~50% that of SV-473.2 SV-269 is a leucine zipper motif which specifically binds Sendai virions and inhibits virus-mediated hemolysis ( 43).	bind
26002	9	7084	7	NULL	NULL	0	NULL	virus	NULL		mediates	NULL				hemolysis	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_42_27182_s_169	9765238	2 SV-150, composed of amino acids 150-186, is an elongated version of the biologically inactive SV-163 peptide ( 32) that inhibits virus-mediated erythrocyte hemolysis at doses ~50% that of SV-473.2 SV-269 is a leucine zipper motif which specifically binds Sendai virions and inhibits virus-mediated hemolysis ( 43).	bind
26003	10	7084	7	NULL	NULL	0	NULL	statement 8	NULL		inhibits	NULL				statement 9	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_42_27182_s_169	9765238	2 SV-150, composed of amino acids 150-186, is an elongated version of the biologically inactive SV-163 peptide ( 32) that inhibits virus-mediated erythrocyte hemolysis at doses ~50% that of SV-473.2 SV-269 is a leucine zipper motif which specifically binds Sendai virions and inhibits virus-mediated hemolysis ( 43).	bind
21975	1	7086	6	13	NULL	NULL	NULL	A6c134 TCR	GP		bind					HLA A2 antigen	Chemical		LLF-GYPVYV		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_3_1882_s_245	15531581	2 The A6c134 TCR binds to HLA A2-LLF-GYPVYV antigen with a half-life of 3900s and can stain cells pulsed with as little as 10 - 8M antigen.	bind
26009	1	7086	7	10	NULL	0	NULL	A6c134 TCR	NULL		binds to	NULL				HLA A2 antigen	NULL		LLF-GYPVYV		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_3_1882_s_245	15531581	2 The A6c134 TCR binds to HLA A2-LLF-GYPVYV antigen with a half-life of 3900s and can stain cells pulsed with as little as 10 - 8M antigen.	bind
21976	1	7093	6	13	NULL	NULL	NULL	Prs a 1	GP		form		may	chitin binding motif		IgE epitope	GP	cross-reactive			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_43_28091_s_217	9774427	2 The amino acid sequence similarity between the major latex allergen hevein and the N-terminal portion of Prs a 1 suggests that the chitin-binding motif of Prs a 1 may form an important cross-reactive IgE epitope.	bind
21977	2	7093	6	13	NULL	NULL	NULL	hevein	GP	amino acid sequence of	is similar to					Prs a 1 	GP		N-terminal portion		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_43_28091_s_217	9774427	2 The amino acid sequence similarity between the major latex allergen hevein and the N-terminal portion of Prs a 1 suggests that the chitin-binding motif of Prs a 1 may form an important cross-reactive IgE epitope.	bind
46439	3	7093	6	10	NULL	0	NULL	hevein	NULL		is a type of	NULL				latex allergen	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_43_28091_s_217	9774427	2 The amino acid sequence similarity between the major latex allergen hevein and the N-terminal portion of Prs a 1 suggests that the chitin-binding motif of Prs a 1 may form an important cross-reactive IgE epitope.	bind
26011	1	7093	7	NULL	NULL	0	NULL	Prs a 1	NULL		forms	NULL		chitin-binding motif 		IgE epitope	NULL	cross-reactive 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_43_28091_s_217	9774427	2 The amino acid sequence similarity between the major latex allergen hevein and the N-terminal portion of Prs a 1 suggests that the chitin-binding motif of Prs a 1 may form an important cross-reactive IgE epitope.	bind
21978	1	7094	6	13	NULL	NULL	NULL	gp59	GP		bind					statement 6	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_50_49839_s_27	14500719	2 The binding of gp59 to gp32 coated DNA facilitates the loading of a hexameric helicase with the lagging DNA strand passing through the center of a complex of the helicase and gp59 ( ).	bind
22213	2	7094	6	13	NULL	NULL	NULL	hexameric helicase	GP		forms a complex with					gp59	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_50_49839_s_27	14500719	2 The binding of gp59 to gp32 coated DNA facilitates the loading of a hexameric helicase with the lagging DNA strand passing through the center of a complex of the helicase and gp59 ( ).	bind
22214	3	7094	6	13	NULL	NULL	NULL	lagging DNA strand	NucleicAcid		passes through					statement 2	Process	center of 			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_50_49839_s_27	14500719	2 The binding of gp59 to gp32 coated DNA facilitates the loading of a hexameric helicase with the lagging DNA strand passing through the center of a complex of the helicase and gp59 ( ).	bind
22215	4	7094	6	13	NULL	NULL	NULL	statement 1	Process		facilitates					hexameric helicase	GP	loading of 			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_50_49839_s_27	14500719	2 The binding of gp59 to gp32 coated DNA facilitates the loading of a hexameric helicase with the lagging DNA strand passing through the center of a complex of the helicase and gp59 ( ).	bind
22216	5	7094	6	13	NULL	NULL	NULL	statement 1	Process		facilitates					statement 3	Process	loading of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_50_49839_s_27	14500719	2 The binding of gp59 to gp32 coated DNA facilitates the loading of a hexameric helicase with the lagging DNA strand passing through the center of a complex of the helicase and gp59 ( ).	bind
46440	6	7094	6	13	NULL	NULL	NULL	DNA	NucleicAcid		is coated with					gp32	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_50_49839_s_27	14500719	2 The binding of gp59 to gp32 coated DNA facilitates the loading of a hexameric helicase with the lagging DNA strand passing through the center of a complex of the helicase and gp59 ( ).	bind
26012	1	7094	7	10	NULL	0	NULL	gp59	NULL		binds	NULL				statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_50_49839_s_27	14500719	2 The binding of gp59 to gp32 coated DNA facilitates the loading of a hexameric helicase with the lagging DNA strand passing through the center of a complex of the helicase and gp59 ( ).	bind
26013	2	7094	7	NULL	NULL	0	NULL	statement 1	NULL		facilitate	NULL				hexameric helicase	NULL	loading of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_50_49839_s_27	14500719	2 The binding of gp59 to gp32 coated DNA facilitates the loading of a hexameric helicase with the lagging DNA strand passing through the center of a complex of the helicase and gp59 ( ).	bind
26014	4	7094	7	NULL	NULL	0	NULL	lagging DNA strand	NULL		pass through 	NULL				statement 3	NULL	the center of the complex of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_50_49839_s_27	14500719	2 The binding of gp59 to gp32 coated DNA facilitates the loading of a hexameric helicase with the lagging DNA strand passing through the center of a complex of the helicase and gp59 ( ).	bind
26015	3	7094	7	NULL	NULL	0	NULL	gp59	NULL		complex with	NULL				helicase	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_50_49839_s_27	14500719	2 The binding of gp59 to gp32 coated DNA facilitates the loading of a hexameric helicase with the lagging DNA strand passing through the center of a complex of the helicase and gp59 ( ).	bind
46441	5	7094	7	10	NULL	0	NULL	DNA	NULL		is coated with	NULL				gp32	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_50_49839_s_27	14500719	2 The binding of gp59 to gp32 coated DNA facilitates the loading of a hexameric helicase with the lagging DNA strand passing through the center of a complex of the helicase and gp59 ( ).	bind
22059	1	7095	6	13	NULL	NULL	NULL	polyubiquitin	GP		bind					p97 complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_37_34774_s_274	12813030	2 The binding of polyubiquitin to the p97 complex is also  consistent with it being the immediate downstream component.	bind
26016	1	7095	7	NULL	NULL	0	NULL	polyubiquitin	NULL		binds	NULL				p97 complex	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_34774_s_274	12813030	2 The binding of polyubiquitin to the p97 complex is also  consistent with it being the immediate downstream component.	bind
22062	1	7096	6	13	NULL	NULL	NULL				bind			rC domain		fibronectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_11_7473_s_226	9054449	2 The binding of rC domain to fibronectin and potentially to heparan sulfate proteoglycans reveals additional extracellular or pericellular matrix components that may serve as anchors to sequester gelatinase A in tissues and to the cell surface.	bind
22064	2	7096	6	13	NULL	NULL	NULL				bind		potentially	rC domain		heparan sulfate proteoglycans	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_11_7473_s_226	9054449	2 The binding of rC domain to fibronectin and potentially to heparan sulfate proteoglycans reveals additional extracellular or pericellular matrix components that may serve as anchors to sequester gelatinase A in tissues and to the cell surface.	bind
22217	3	7096	6	13	NULL	NULL	NULL	gelatinase A	GP		sequestered in					tissues	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_11_7473_s_226	9054449	2 The binding of rC domain to fibronectin and potentially to heparan sulfate proteoglycans reveals additional extracellular or pericellular matrix components that may serve as anchors to sequester gelatinase A in tissues and to the cell surface.	bind
22218	4	7096	6	13	NULL	NULL	NULL	gelatinase A	GP		sequestered to					cell surface	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_11_7473_s_226	9054449	2 The binding of rC domain to fibronectin and potentially to heparan sulfate proteoglycans reveals additional extracellular or pericellular matrix components that may serve as anchors to sequester gelatinase A in tissues and to the cell surface.	bind
22219	5	7096	6	13	NULL	NULL	NULL	extracellular matrix components	CellComponent		serve as anchors for		may			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_11_7473_s_226	9054449	2 The binding of rC domain to fibronectin and potentially to heparan sulfate proteoglycans reveals additional extracellular or pericellular matrix components that may serve as anchors to sequester gelatinase A in tissues and to the cell surface.	bind
22220	6	7096	6	NULL	NULL	0	NULL	pericellular matrix components	NULL		serve as anchors for	NULL	may			statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_11_7473_s_226	9054449	2 The binding of rC domain to fibronectin and potentially to heparan sulfate proteoglycans reveals additional extracellular or pericellular matrix components that may serve as anchors to sequester gelatinase A in tissues and to the cell surface.	bind
22221	7	7096	6	NULL	NULL	0	NULL	extracellular matrix components	NULL		serve as anchors for	NULL	may			statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_11_7473_s_226	9054449	2 The binding of rC domain to fibronectin and potentially to heparan sulfate proteoglycans reveals additional extracellular or pericellular matrix components that may serve as anchors to sequester gelatinase A in tissues and to the cell surface.	bind
22222	8	7096	6	NULL	NULL	0	NULL	pericellular matrix components	NULL		serve as anchors for	NULL	may			statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_11_7473_s_226	9054449	2 The binding of rC domain to fibronectin and potentially to heparan sulfate proteoglycans reveals additional extracellular or pericellular matrix components that may serve as anchors to sequester gelatinase A in tissues and to the cell surface.	bind
26017	1	7096	7	NULL	NULL	0	NULL		NULL		binds	NULL		rC domain		fibronectin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_11_7473_s_226	9054449	2 The binding of rC domain to fibronectin and potentially to heparan sulfate proteoglycans reveals additional extracellular or pericellular matrix components that may serve as anchors to sequester gelatinase A in tissues and to the cell surface.	bind
26018	2	7096	7	NULL	NULL	0	NULL		NULL		bind	NULL	potentially	rC domain		heparan sulfate proteoglycans 	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_11_7473_s_226	9054449	2 The binding of rC domain to fibronectin and potentially to heparan sulfate proteoglycans reveals additional extracellular or pericellular matrix components that may serve as anchors to sequester gelatinase A in tissues and to the cell surface.	bind
26019	3	7096	7	NULL	NULL	0	NULL	gelatinase A 			sequestered in					tissues					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_11_7473_s_226	9054449	2 The binding of rC domain to fibronectin and potentially to heparan sulfate proteoglycans reveals additional extracellular or pericellular matrix components that may serve as anchors to sequester gelatinase A in tissues and to the cell surface.	bind
26020	4	7096	7	NULL	NULL	0	NULL	gelatinase A			sequestered in					cell surface					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_11_7473_s_226	9054449	2 The binding of rC domain to fibronectin and potentially to heparan sulfate proteoglycans reveals additional extracellular or pericellular matrix components that may serve as anchors to sequester gelatinase A in tissues and to the cell surface.	bind
26021	5	7096	7	NULL	NULL	0	NULL	extracellular matrix components			serve as anchor to		may			statement 3					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_11_7473_s_226	9054449	2 The binding of rC domain to fibronectin and potentially to heparan sulfate proteoglycans reveals additional extracellular or pericellular matrix components that may serve as anchors to sequester gelatinase A in tissues and to the cell surface.	bind
26022	6	7096	7	NULL	NULL	0	NULL	extracellular matrix components			serve as anchor to		may			statement 4					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_11_7473_s_226	9054449	2 The binding of rC domain to fibronectin and potentially to heparan sulfate proteoglycans reveals additional extracellular or pericellular matrix components that may serve as anchors to sequester gelatinase A in tissues and to the cell surface.	bind
26023	7	7096	7	NULL	NULL	0	NULL	pericellular matrix components			serve as anchor to		may			statement 3					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_11_7473_s_226	9054449	2 The binding of rC domain to fibronectin and potentially to heparan sulfate proteoglycans reveals additional extracellular or pericellular matrix components that may serve as anchors to sequester gelatinase A in tissues and to the cell surface.	bind
26024	8	7096	7	10	NULL	0	NULL	pericellular matrix components			serve as anchor to		may			statement 4					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_11_7473_s_226	9054449	2 The binding of rC domain to fibronectin and potentially to heparan sulfate proteoglycans reveals additional extracellular or pericellular matrix components that may serve as anchors to sequester gelatinase A in tissues and to the cell surface.	bind
22065	1	7097	6	13	NULL	NULL	NULL	Wnt ligands	GP		bind					cell-surface receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_3_1381_s_12	16293629	2 The binding of Wnt ligands to cell-surface receptors leads to the activation of the intracellular protein Dishevelled.	bind
22066	2	7097	6	13	NULL	NULL	NULL	statement 1	Process		leads to					Dishevelled	GP	activation of 			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_3_1381_s_12	16293629	2 The binding of Wnt ligands to cell-surface receptors leads to the activation of the intracellular protein Dishevelled.	bind
46442	3	7097	6	13	NULL	NULL	NULL	Dishevelled	GP		is a type of					intracellular protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_3_1381_s_12	16293629	2 The binding of Wnt ligands to cell-surface receptors leads to the activation of the intracellular protein Dishevelled.	bind
26025	1	7097	7	NULL	NULL	0	NULL	Wnt ligands	NULL		binds	NULL				cell-surface receptors	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_3_1381_s_12	16293629	2 The binding of Wnt ligands to cell-surface receptors leads to the activation of the intracellular protein Dishevelled.	bind
26026	2	7097	7	10	NULL	0	NULL	statement 1	NULL		leads to	NULL				Dishevelled	NULL	activation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_3_1381_s_12	16293629	2 The binding of Wnt ligands to cell-surface receptors leads to the activation of the intracellular protein Dishevelled.	bind
46443	3	7097	7	10	NULL	0	NULL	Dishevelled	NULL		is a type of	NULL				intracellular protein	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_3_1381_s_12	16293629	2 The binding of Wnt ligands to cell-surface receptors leads to the activation of the intracellular protein Dishevelled.	bind
22067	1	7098	6	13	NULL	NULL	NULL				bind				CArG box element	SRF	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_3_1511_s_260	9430690	2 The CArG box element is known to bind to SRF or related factors; however, the precise role of SRF transcription factors in smooth muscle-specific gene expression remains to be explored.	bind
22069	2	7098	6	13	NULL	NULL	NULL	SRF	GP		plays a role in		may			smooth muscle-specific gene 	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_3_1511_s_260	9430690	2 The CArG box element is known to bind to SRF or related factors; however, the precise role of SRF transcription factors in smooth muscle-specific gene expression remains to be explored.	bind
27030	3	7098	6	13	NULL	NULL	NULL	SRF	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_3_1511_s_260	9430690	2 The CArG box element is known to bind to SRF or related factors; however, the precise role of SRF transcription factors in smooth muscle-specific gene expression remains to be explored.	bind
26027	1	7098	7	NULL	NULL	0	NULL		NULL		binds to	NULL			CArG box element	SRF	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_3_1511_s_260	9430690	2 The CArG box element is known to bind to SRF or related factors; however, the precise role of SRF transcription factors in smooth muscle-specific gene expression remains to be explored.	bind
26028	2	7098	7	NULL	NULL	0	NULL	SRF	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_3_1511_s_260	9430690	2 The CArG box element is known to bind to SRF or related factors; however, the precise role of SRF transcription factors in smooth muscle-specific gene expression remains to be explored.	bind
28506	3	7098	7	10	NULL	0	NULL	SRF	NULL		plays a role in	NULL	may			smooth muscle-specific gene 	NULL	expression of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_3_1511_s_260	9430690	2 The CArG box element is known to bind to SRF or related factors; however, the precise role of SRF transcription factors in smooth muscle-specific gene expression remains to be explored.	bind
22070	1	7100	6	13	NULL	NULL	NULL	NapC	GP		bind					hemes	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_44_28785_s_145	9786877	2 The combined approach of UV-visible, EPR, MCD, and redox potentiometry provides unambiguous evidence that NapC binds four hemes, all of which are low spin and  bis-His-ligated in the ferric state.	bind
26033	1	7100	7	NULL	NULL	0	NULL	NapC	NULL		binds	NULL				heme	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_44_28785_s_145	9786877	2 The combined approach of UV-visible, EPR, MCD, and redox potentiometry provides unambiguous evidence that NapC binds four hemes, all of which are low spin and  bis-His-ligated in the ferric state.	bind
22073	1	7101	6	13	NULL	NULL	NULL	insulin	GP		bind				CRE	winged helix-like proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_29_18499_s_247	9660819	2 The cross-competition between the insulin CRE and G3B indicates that the winged helix-like proteins binding to the insulin CRE are the same as those binding to domain B of the G3 enhancer element of the glucagon gene.	bind
22074	2	7101	6	13	NULL	NULL	NULL	glucagon gene	GP		bind				domain B of G3 enhancer	winged helix-like proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_29_18499_s_247	9660819	2 The cross-competition between the insulin CRE and G3B indicates that the winged helix-like proteins binding to the insulin CRE are the same as those binding to domain B of the G3 enhancer element of the glucagon gene.	bind
27031	3	7101	6	13	NULL	NULL	NULL	statement 1	Process		competes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_29_18499_s_247	9660819	2 The cross-competition between the insulin CRE and G3B indicates that the winged helix-like proteins binding to the insulin CRE are the same as those binding to domain B of the G3 enhancer element of the glucagon gene.	bind
26035	1	7101	7	NULL	NULL	0	NULL	winged helix-like proteins	NULL		bind	NULL				insulin	NULL			CRE	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_29_18499_s_247	9660819	2 The cross-competition between the insulin CRE and G3B indicates that the winged helix-like proteins binding to the insulin CRE are the same as those binding to domain B of the G3 enhancer element of the glucagon gene.	bind
26036	2	7101	7	NULL	NULL	0	NULL	winged helix-like proteins	NULL		bind	NULL				glucagon gene	NULL			domain B of G3 enhancer	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_29_18499_s_247	9660819	2 The cross-competition between the insulin CRE and G3B indicates that the winged helix-like proteins binding to the insulin CRE are the same as those binding to domain B of the G3 enhancer element of the glucagon gene.	bind
26037	3	7101	7	10	NULL	0	NULL	statement 1	NULL		competes with	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_29_18499_s_247	9660819	2 The cross-competition between the insulin CRE and G3B indicates that the winged helix-like proteins binding to the insulin CRE are the same as those binding to domain B of the G3 enhancer element of the glucagon gene.	bind
22075	1	7103	6	13	NULL	NULL	NULL	Rgt1	GP		does not bind					HXT1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_12_10322_s_110	12527758	2 The data obtained with the ChIP assay indicate that Rgt1 does not bind to the  HXT1 promoter in response to glucose and that it activates  HXT1 gene expression probably by an indirect mechanism.	bind
22076	2	7103	6	13	NULL	NULL	NULL	statement 1	Process		occurs in response to					glucose	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_12_10322_s_110	12527758	2 The data obtained with the ChIP assay indicate that Rgt1 does not bind to the  HXT1 promoter in response to glucose and that it activates  HXT1 gene expression probably by an indirect mechanism.	bind
22077	3	7103	6	13	NULL	NULL	NULL	Rgt1	GP		activates					HXT1	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_12_10322_s_110	12527758	2 The data obtained with the ChIP assay indicate that Rgt1 does not bind to the  HXT1 promoter in response to glucose and that it activates  HXT1 gene expression probably by an indirect mechanism.	bind
26038	1	7103	7	NULL	NULL	0	NULL	Rgt1	NULL		does not bind	NULL				HXT1	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10322_s_110	12527758	2 The data obtained with the ChIP assay indicate that Rgt1 does not bind to the  HXT1 promoter in response to glucose and that it activates  HXT1 gene expression probably by an indirect mechanism.	bind
26039	2	7103	7	NULL	NULL	0	NULL	statement 1	NULL		in response to	NULL				glucose	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10322_s_110	12527758	2 The data obtained with the ChIP assay indicate that Rgt1 does not bind to the  HXT1 promoter in response to glucose and that it activates  HXT1 gene expression probably by an indirect mechanism.	bind
26040	3	7103	7	NULL	NULL	0	NULL	Rgt1	NULL		activates	NULL				HXT1 gene	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10322_s_110	12527758	2 The data obtained with the ChIP assay indicate that Rgt1 does not bind to the  HXT1 promoter in response to glucose and that it activates  HXT1 gene expression probably by an indirect mechanism.	bind
22078	1	7104	6	13	NULL	NULL	NULL	IGFBP-7	GP		bind					IGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_48_30322_s_99	8939990	2 The failure to demonstrate IGFBP-7 binding of IGF by conventional Western ligand blotting methods may be attributable to the loss of structural integrity under denaturing conditions, since binding was observed when blotting was performed with non-denaturing gels.	bind
26041	1	7104	7	NULL	NULL	0	NULL	IGF	NULL		bind	NULL				IGFBP-7	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_48_30322_s_99	8939990	2 The failure to demonstrate IGFBP-7 binding of IGF by conventional Western ligand blotting methods may be attributable to the loss of structural integrity under denaturing conditions, since binding was observed when blotting was performed with non-denaturing gels.	bind
22079	1	7106	6	13	NULL	NULL	NULL	Cbl	GP	phosphorylated	bind			tyrosine		Hck	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_19_14615_s_150	10799548	2 The filter was reprobed with anti-phosphotyrosine antibodies in order to determine if tyrosine-phosphorylated Cbl binds the SH3 domain of Hck in preference to the SH2.	bind
27032	2	7106	6	13	NULL	NULL	NULL	Cbl	GP	phosphorylated	bind			tyrosine		Hck	GP		SH2 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_19_14615_s_150	10799548	2 The filter was reprobed with anti-phosphotyrosine antibodies in order to determine if tyrosine-phosphorylated Cbl binds the SH3 domain of Hck in preference to the SH2.	bind
46444	3	7106	6	13	NULL	NULL	NULL	statement 2	Process		is preferred over					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_19_14615_s_150	10799548	2 The filter was reprobed with anti-phosphotyrosine antibodies in order to determine if tyrosine-phosphorylated Cbl binds the SH3 domain of Hck in preference to the SH2.	bind
26049	1	7106	7	NULL	NULL	0	NULL	Cbl	NULL	phosphorylated	binds	NULL		tyrosine		Hck	NULL		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_19_14615_s_150	10799548	2 The filter was reprobed with anti-phosphotyrosine antibodies in order to determine if tyrosine-phosphorylated Cbl binds the SH3 domain of Hck in preference to the SH2.	bind
26051	2	7106	7	NULL	NULL	0	NULL	Cbl	NULL	phosphorylated	binds	NULL		tyrosine		Hck	NULL		SH2 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_19_14615_s_150	10799548	2 The filter was reprobed with anti-phosphotyrosine antibodies in order to determine if tyrosine-phosphorylated Cbl binds the SH3 domain of Hck in preference to the SH2.	bind
26054	3	7106	7	NULL	NULL	0	NULL	statement 2	NULL		is preferred than	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_19_14615_s_150	10799548	2 The filter was reprobed with anti-phosphotyrosine antibodies in order to determine if tyrosine-phosphorylated Cbl binds the SH3 domain of Hck in preference to the SH2.	bind
22080	1	7107	6	13	NULL	NULL	NULL	nuclear protein	GP	transport of	is regulated at 		differentially			NLS recognition step	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_42_26375_s_196	9334211	2 The findings herein suggest that nuclear protein transport is differentially regulated at the NLS recognition step through the expression level and/or the controls of NLS binding specificities of NLS receptors in various cells, which, in turn, may lead to the regulation of development or cell differentiation.	bind
22081	2	7107	6	13	NULL	NULL	NULL	NLS receptor	GP		bind					NLS	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_42_26375_s_196	9334211	2 The findings herein suggest that nuclear protein transport is differentially regulated at the NLS recognition step through the expression level and/or the controls of NLS binding specificities of NLS receptors in various cells, which, in turn, may lead to the regulation of development or cell differentiation.	bind
22082	3	7107	6	13	NULL	NULL	NULL	statement 1	Process		occurs by					statement 2	Process	control of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_42_26375_s_196	9334211	2 The findings herein suggest that nuclear protein transport is differentially regulated at the NLS recognition step through the expression level and/or the controls of NLS binding specificities of NLS receptors in various cells, which, in turn, may lead to the regulation of development or cell differentiation.	bind
22083	4	7107	6	13	NULL	NULL	NULL	statement 3	Process		lead to		may			development	Process	regulation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_42_26375_s_196	9334211	2 The findings herein suggest that nuclear protein transport is differentially regulated at the NLS recognition step through the expression level and/or the controls of NLS binding specificities of NLS receptors in various cells, which, in turn, may lead to the regulation of development or cell differentiation.	bind
22084	5	7107	6	13	NULL	NULL	NULL	statement 3	Process		lead to 		may			cell differentiation	Process	regulation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_42_26375_s_196	9334211	2 The findings herein suggest that nuclear protein transport is differentially regulated at the NLS recognition step through the expression level and/or the controls of NLS binding specificities of NLS receptors in various cells, which, in turn, may lead to the regulation of development or cell differentiation.	bind
26055	1	7107	7	NULL	NULL	0	NULL	nuclear protein 	NULL	transport of	regulated at	NULL	differentially			NLS recognition step	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_42_26375_s_196	9334211	2 The findings herein suggest that nuclear protein transport is differentially regulated at the NLS recognition step through the expression level and/or the controls of NLS binding specificities of NLS receptors in various cells, which, in turn, may lead to the regulation of development or cell differentiation.	bind
26057	3	7107	7	10	NULL	0	NULL	NLS	NULL		bind	NULL				NLS receptors	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_42_26375_s_196	9334211	2 The findings herein suggest that nuclear protein transport is differentially regulated at the NLS recognition step through the expression level and/or the controls of NLS binding specificities of NLS receptors in various cells, which, in turn, may lead to the regulation of development or cell differentiation.	bind
26058	4	7107	7	NULL	NULL	0	NULL	statement 1	NULL		occurs through	NULL				statement 3	NULL	control of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_42_26375_s_196	9334211	2 The findings herein suggest that nuclear protein transport is differentially regulated at the NLS recognition step through the expression level and/or the controls of NLS binding specificities of NLS receptors in various cells, which, in turn, may lead to the regulation of development or cell differentiation.	bind
26059	5	7107	7	NULL	NULL	0	NULL	statement 3	NULL		lead to	NULL	may			development	NULL	regulation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_42_26375_s_196	9334211	2 The findings herein suggest that nuclear protein transport is differentially regulated at the NLS recognition step through the expression level and/or the controls of NLS binding specificities of NLS receptors in various cells, which, in turn, may lead to the regulation of development or cell differentiation.	bind
26060	6	7107	7	NULL	NULL	0	NULL	statement 3	NULL		lead to	NULL	may			cell differentiation	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_42_26375_s_196	9334211	2 The findings herein suggest that nuclear protein transport is differentially regulated at the NLS recognition step through the expression level and/or the controls of NLS binding specificities of NLS receptors in various cells, which, in turn, may lead to the regulation of development or cell differentiation.	bind
22085	1	7108	6	13	NULL	NULL	NULL	heme	Chemical		bind					CYP4A protein	GP		glutamic acid residue on the I-helix		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_12755_s_23	11821421	2 The heme is bound to the CYP4A proteins via a conserved glutamic acid residue on the I-helix of the protein ( 16).	bind
26061	1	7108	7	NULL	NULL	0	NULL	 heme	NULL		binds	NULL				CYP4A proteins	NULL		glutamic acid residue on the I-helix of		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_12755_s_23	11821421	2 The heme is bound to the CYP4A proteins via a conserved glutamic acid residue on the I-helix of the protein ( 16).	bind
22086	1	7109	6	13	NULL	NULL	NULL	pro-IAPP peptide	GP		bind			N-terminal		heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_20_16611_s_136	11145957	2 The heparin binding activity of the N-terminal pro-IAPP peptide therefore does not depend upon any conformational change induced by formation of the disulfide bond.	bind
22087	2	7109	6	13	NULL	NULL	NULL	disulfide bond	Process	formation of	induces					conformational change	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_20_16611_s_136	11145957	2 The heparin binding activity of the N-terminal pro-IAPP peptide therefore does not depend upon any conformational change induced by formation of the disulfide bond.	bind
22088	3	7109	6	13	NULL	NULL	NULL	statement 1	Process		does not depend upon					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_20_16611_s_136	11145957	2 The heparin binding activity of the N-terminal pro-IAPP peptide therefore does not depend upon any conformational change induced by formation of the disulfide bond.	bind
26063	1	7109	7	NULL	NULL	0	NULL	pro-IAPP peptide	NULL		binds	NULL		N-terminal		heparin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_20_16611_s_136	11145957	2 The heparin binding activity of the N-terminal pro-IAPP peptide therefore does not depend upon any conformational change induced by formation of the disulfide bond.	bind
26064	2	7109	7	NULL	NULL	0	NULL	disulfide bond	NULL	 formation of	induce	NULL				conformational change	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_20_16611_s_136	11145957	2 The heparin binding activity of the N-terminal pro-IAPP peptide therefore does not depend upon any conformational change induced by formation of the disulfide bond.	bind
26065	3	7109	7	NULL	NULL	0	NULL	statement 1	NULL		does not depend on	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_20_16611_s_136	11145957	2 The heparin binding activity of the N-terminal pro-IAPP peptide therefore does not depend upon any conformational change induced by formation of the disulfide bond.	bind
22089	1	7110	6	13	NULL	NULL	NULL	TGF-beta1	GP	125I	bind					TGF-beta receptors	GP				NULL	mink lung epithelial cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_33_20572_s_35	9252371	2 The IC50 values of TGF-beta1 and TGF-beta3 peptide antagonists for inhibiting 125I-TGF-beta1 (0.1 nM) binding to TGF-beta receptors in mink lung epithelial cells are ~1-2 and ~20-30 muM, respectively.	bind
22090	2	7110	6	13	NULL	NULL	NULL	TGF-beta1 peptide antagonist	Chemical		inhibit					statement 1	Process				NULL	mink lung epithelial cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_33_20572_s_35	9252371	2 The IC50 values of TGF-beta1 and TGF-beta3 peptide antagonists for inhibiting 125I-TGF-beta1 (0.1 nM) binding to TGF-beta receptors in mink lung epithelial cells are ~1-2 and ~20-30 muM, respectively.	bind
22091	3	7110	6	13	NULL	NULL	NULL	TGF-beta3 peptide antagonist	Chemical		inhibit					statement 1	Process				NULL	mink lung epithelial cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_33_20572_s_35	9252371	2 The IC50 values of TGF-beta1 and TGF-beta3 peptide antagonists for inhibiting 125I-TGF-beta1 (0.1 nM) binding to TGF-beta receptors in mink lung epithelial cells are ~1-2 and ~20-30 muM, respectively.	bind
26066	1	7110	7	NULL	NULL	0	NULL	TGF-beta1 	NULL	125I	bind	NULL				TGF-beta receptors	NULL				NULL	mink lung epithelial cells	0	NULL	NULL	NULL	gw60_jbiolchem_272_33_20572_s_35	9252371	2 The IC50 values of TGF-beta1 and TGF-beta3 peptide antagonists for inhibiting 125I-TGF-beta1 (0.1 nM) binding to TGF-beta receptors in mink lung epithelial cells are ~1-2 and ~20-30 muM, respectively.	bind
26067	2	7110	7	10	NULL	0	NULL	TGF-beta1 peptide antagonist	NULL		inhibits	NULL				statement 1	NULL				NULL	mink lung epithelial cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_33_20572_s_35	9252371	2 The IC50 values of TGF-beta1 and TGF-beta3 peptide antagonists for inhibiting 125I-TGF-beta1 (0.1 nM) binding to TGF-beta receptors in mink lung epithelial cells are ~1-2 and ~20-30 muM, respectively.	bind
26068	3	7110	7	10	NULL	0	NULL	TGF-beta3 peptide antagonist	NULL		inhibits	NULL				statement 1	NULL				NULL	mink lung epithelial cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_33_20572_s_35	9252371	2 The IC50 values of TGF-beta1 and TGF-beta3 peptide antagonists for inhibiting 125I-TGF-beta1 (0.1 nM) binding to TGF-beta receptors in mink lung epithelial cells are ~1-2 and ~20-30 muM, respectively.	bind
22092	1	7111	6	13	NULL	NULL	NULL	hypertonicity			increases					TonEBP	GP	activity of 			NULL	HeLa cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_32_20615_s_208	9685419	2 The increase in TonEBP activity in HeLa cells in response to hypertonicity (Fig.  4) predicts that there should be a parallel increase in binding of TonEBP to the SMIT TonEs.	bind
22093	2	7111	6	13	NULL	NULL	NULL	TonEBP	GP		bind					SMIT TonE	GP				NULL	HeLa cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_32_20615_s_208	9685419	2 The increase in TonEBP activity in HeLa cells in response to hypertonicity (Fig.  4) predicts that there should be a parallel increase in binding of TonEBP to the SMIT TonEs.	bind
22094	3	7111	6	13	NULL	NULL	NULL	statement 1	Process		increases		may;;partially			statement 2	Process				NULL	HeLa cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_32_20615_s_208	9685419	2 The increase in TonEBP activity in HeLa cells in response to hypertonicity (Fig.  4) predicts that there should be a parallel increase in binding of TonEBP to the SMIT TonEs.	bind
26069	1	7111	7	10	NULL	0	NULL	TonEBP	NULL		binds	NULL				SMIT TonEs	NULL				NULL	HeLa cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_32_20615_s_208	9685419	2 The increase in TonEBP activity in HeLa cells in response to hypertonicity (Fig.  4) predicts that there should be a parallel increase in binding of TonEBP to the SMIT TonEs.	bind
26070	2	7111	7	NULL	NULL	0	NULL	hypertonicity 	NULL		increase	NULL				TonEBP	NULL	activity of			NULL	HeLa cells	0	NULL	NULL	NULL	gw60_jbiolchem_273_32_20615_s_208	9685419	2 The increase in TonEBP activity in HeLa cells in response to hypertonicity (Fig.  4) predicts that there should be a parallel increase in binding of TonEBP to the SMIT TonEs.	bind
26071	3	7111	7	10	NULL	0	NULL	statement 1	NULL		increases	NULL	may;;partially			statement 1	NULL				NULL	HeLa cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_32_20615_s_208	9685419	2 The increase in TonEBP activity in HeLa cells in response to hypertonicity (Fig.  4) predicts that there should be a parallel increase in binding of TonEBP to the SMIT TonEs.	bind
22095	1	7112	6	13	NULL	NULL	NULL	apoACP	GP		bind			S36T		AcpS	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_2_959_s_250	10625633	2 The introduction of the gamma-CH3 in S36T apoACP blocked the conversion of this protein to the holo form, but the binding of S36T apoACP by AcpS may induce an allosteric change in the homodimeric enzyme that relieves substrate inhibition by apoACP.	bind
22096	2	7112	6	13	NULL	NULL	NULL	statement 1	Process		induce		may			homodimeric enzyme	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_2_959_s_250	10625633	2 The introduction of the gamma-CH3 in S36T apoACP blocked the conversion of this protein to the holo form, but the binding of S36T apoACP by AcpS may induce an allosteric change in the homodimeric enzyme that relieves substrate inhibition by apoACP.	bind
22225	3	7112	6	13	NULL	NULL	NULL				introduced to			gamma-CH3		apoACP	GP		S36T		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_2_959_s_250	10625633	2 The introduction of the gamma-CH3 in S36T apoACP blocked the conversion of this protein to the holo form, but the binding of S36T apoACP by AcpS may induce an allosteric change in the homodimeric enzyme that relieves substrate inhibition by apoACP.	bind
22226	4	7112	6	13	NULL	NULL	NULL	apoACP	GP		converted to					holo form	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_2_959_s_250	10625633	2 The introduction of the gamma-CH3 in S36T apoACP blocked the conversion of this protein to the holo form, but the binding of S36T apoACP by AcpS may induce an allosteric change in the homodimeric enzyme that relieves substrate inhibition by apoACP.	bind
22227	5	7112	6	13	NULL	NULL	NULL	statement 3	Process		blocks 					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_2_959_s_250	10625633	2 The introduction of the gamma-CH3 in S36T apoACP blocked the conversion of this protein to the holo form, but the binding of S36T apoACP by AcpS may induce an allosteric change in the homodimeric enzyme that relieves substrate inhibition by apoACP.	bind
22228	6	7112	6	13	NULL	NULL	NULL	statement 2	Process		relieves					apoACP	GP	substrate inhibition by			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_2_959_s_250	10625633	2 The introduction of the gamma-CH3 in S36T apoACP blocked the conversion of this protein to the holo form, but the binding of S36T apoACP by AcpS may induce an allosteric change in the homodimeric enzyme that relieves substrate inhibition by apoACP.	bind
27033	7	7112	6	13	NULL	NULL	NULL	apoACP	GP		inhibits					homodimeric enzyme	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_2_959_s_250	10625633	2 The introduction of the gamma-CH3 in S36T apoACP blocked the conversion of this protein to the holo form, but the binding of S36T apoACP by AcpS may induce an allosteric change in the homodimeric enzyme that relieves substrate inhibition by apoACP.	bind
27034	8	7112	6	13	NULL	NULL	NULL	statement 4	Process		relieves					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_2_959_s_250	10625633	2 The introduction of the gamma-CH3 in S36T apoACP blocked the conversion of this protein to the holo form, but the binding of S36T apoACP by AcpS may induce an allosteric change in the homodimeric enzyme that relieves substrate inhibition by apoACP.	bind
26072	1	7112	7	10	NULL	0	NULL		NULL		added to	NULL		gamma-CH3		apoACP	NULL		S36T		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_2_959_s_250	10625633	2 The introduction of the gamma-CH3 in S36T apoACP blocked the conversion of this protein to the holo form, but the binding of S36T apoACP by AcpS may induce an allosteric change in the homodimeric enzyme that relieves substrate inhibition by apoACP.	bind
26073	2	7112	7	10	NULL	0	NULL	statement 1	NULL		blocks	NULL				statement 7	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_2_959_s_250	10625633	2 The introduction of the gamma-CH3 in S36T apoACP blocked the conversion of this protein to the holo form, but the binding of S36T apoACP by AcpS may induce an allosteric change in the homodimeric enzyme that relieves substrate inhibition by apoACP.	bind
26074	3	7112	7	10	NULL	0	NULL	AcpS	NULL		bind	NULL				apoACP	NULL		S36T		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_2_959_s_250	10625633	2 The introduction of the gamma-CH3 in S36T apoACP blocked the conversion of this protein to the holo form, but the binding of S36T apoACP by AcpS may induce an allosteric change in the homodimeric enzyme that relieves substrate inhibition by apoACP.	bind
26075	4	7112	7	NULL	NULL	0	NULL	statement 3	NULL		induce	NULL				homodimeric enzyme	NULL	allosteric change in			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_2_959_s_250	10625633	2 The introduction of the gamma-CH3 in S36T apoACP blocked the conversion of this protein to the holo form, but the binding of S36T apoACP by AcpS may induce an allosteric change in the homodimeric enzyme that relieves substrate inhibition by apoACP.	bind
26076	5	7112	7	NULL	NULL	0	NULL	apoACP	NULL		inhibits	NULL				homodimeric enzyme	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_2_959_s_250	10625633	2 The introduction of the gamma-CH3 in S36T apoACP blocked the conversion of this protein to the holo form, but the binding of S36T apoACP by AcpS may induce an allosteric change in the homodimeric enzyme that relieves substrate inhibition by apoACP.	bind
28513	6	7112	7	NULL	NULL	0	NULL	statement 4	NULL		relieves	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_2_959_s_250	10625633	2 The introduction of the gamma-CH3 in S36T apoACP blocked the conversion of this protein to the holo form, but the binding of S36T apoACP by AcpS may induce an allosteric change in the homodimeric enzyme that relieves substrate inhibition by apoACP.	bind
46445	7	7112	7	10	NULL	0	NULL	apoACP	NULL		is converted to	NULL				holo form	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_2_959_s_250	10625633	2 The introduction of the gamma-CH3 in S36T apoACP blocked the conversion of this protein to the holo form, but the binding of S36T apoACP by AcpS may induce an allosteric change in the homodimeric enzyme that relieves substrate inhibition by apoACP.	bind
22097	1	7113	6	13	NULL	NULL	NULL	H3	GP		is methylated in			Lys 9		G9a / ES cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_17_14996_s_107	12586828	2 The level of H3 Lys-9 methylation of the PWS-IC in  G9a /  ES cells is reduced to ~30% of that observed in  G9a +/+ ES cells.	bind
22098	2	7113	6	13	NULL	NULL	NULL	H3	GP		is methylated in			Lys-9		G9a +/+ ES cells.	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_17_14996_s_107	12586828	2 The level of H3 Lys-9 methylation of the PWS-IC in  G9a /  ES cells is reduced to ~30% of that observed in  G9a +/+ ES cells.	bind
26138	3	7113	6	13	NULL	NULL	NULL	statement 1	Process	level of	is less than					statement 2	Process	level of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_17_14996_s_107	12586828	2 The level of H3 Lys-9 methylation of the PWS-IC in  G9a /  ES cells is reduced to ~30% of that observed in  G9a +/+ ES cells.	bind
26321	1	7113	7	NULL	NULL	0	NULL	H3	NULL		is methylated in	NULL		Lys-9		G9a / ES cells	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_17_14996_s_107	12586828	2 The level of H3 Lys-9 methylation of the PWS-IC in  G9a /  ES cells is reduced to ~30% of that observed in  G9a +/+ ES cells.	bind
26326	2	7113	7	NULL	NULL	0	NULL	H3	NULL		is methylated in	NULL		Lys-9		G9a +/+ ES cells	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_17_14996_s_107	12586828	2 The level of H3 Lys-9 methylation of the PWS-IC in  G9a /  ES cells is reduced to ~30% of that observed in  G9a +/+ ES cells.	bind
26327	3	7113	7	NULL	NULL	0	NULL	statement 1	NULL	levels of	is less than	NULL				statement 2	NULL	levels of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_17_14996_s_107	12586828	2 The level of H3 Lys-9 methylation of the PWS-IC in  G9a /  ES cells is reduced to ~30% of that observed in  G9a +/+ ES cells.	bind
22229	1	7114	6	13	NULL	NULL	NULL	alpha3beta1 integrin	GP	melanoma cell	bind					alpha1(IV)	GP		531-543		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_16_14321_s_21	12574156	2 The melanoma cell alpha3beta1 integrin binds to alpha1(IV)531-543 ( ,  ,  ).	bind
26079	1	7114	7	NULL	NULL	0	NULL	alpha3beta1 integrin	NULL	melanoma cell	binds to	NULL				 alpha1(IV)	NULL		531-543		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_16_14321_s_21	12574156	2 The melanoma cell alpha3beta1 integrin binds to alpha1(IV)531-543 ( ,  ,  ).	bind
22468	1	7115	6	13	NULL	NULL	NULL	4E-BP1	GP		bind					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_52_32779_s_151	9407052	2 The observation that overexpression of a phosphorylation-resistant mutant of eIF2alpha reduces the extent of inhibition of protein synthesis seen during heat shock supports this idea ( 62,  63), although the fact that such protection was only partial is consistent with the hypothesis that other distinct mechanisms ( e.g. the enhanced binding of 4E-BP1 to eIF4E) may also operate to reduce translation rates under this condition.	bind
23104	2	7115	6	13	NULL	NULL	NULL	eIF2alpha	GP	overexpression of;;phosphorylation-resistant mutant of	reduces					protein synthesis	Process	inhibiton of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_52_32779_s_151	9407052	2 The observation that overexpression of a phosphorylation-resistant mutant of eIF2alpha reduces the extent of inhibition of protein synthesis seen during heat shock supports this idea ( 62,  63), although the fact that such protection was only partial is consistent with the hypothesis that other distinct mechanisms ( e.g. the enhanced binding of 4E-BP1 to eIF4E) may also operate to reduce translation rates under this condition.	bind
26080	1	7115	7	10	NULL	0	NULL	eIF2alpha	NULL	overexpression of;;phosphorylation-resistant mutant of	reduces	NULL				protein synthesis	NULL	inhibition of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_52_32779_s_151	9407052	2 The observation that overexpression of a phosphorylation-resistant mutant of eIF2alpha reduces the extent of inhibition of protein synthesis seen during heat shock supports this idea ( 62,  63), although the fact that such protection was only partial is consistent with the hypothesis that other distinct mechanisms ( e.g. the enhanced binding of 4E-BP1 to eIF4E) may also operate to reduce translation rates under this condition.	bind
26081	2	7115	7	NULL	NULL	0	NULL	4E-BP1	NULL		bind	NULL				eIF4E	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_52_32779_s_151	9407052	2 The observation that overexpression of a phosphorylation-resistant mutant of eIF2alpha reduces the extent of inhibition of protein synthesis seen during heat shock supports this idea ( 62,  63), although the fact that such protection was only partial is consistent with the hypothesis that other distinct mechanisms ( e.g. the enhanced binding of 4E-BP1 to eIF4E) may also operate to reduce translation rates under this condition.	bind
22230	1	7116	6	13	NULL	NULL	NULL	p50 homodimer	GP		bind		weakly			IkappaBalpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29840_s_134	10882738	2 The p50 homodimer binds IkappaBalpha weakly with an equilibrium dissociation constant of 218 nM.	bind
26082	1	7116	7	NULL	NULL	0	NULL	p50 homodimer	NULL		binds	NULL	weakly			IkappaBalpha	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29840_s_134	10882738	2 The p50 homodimer binds IkappaBalpha weakly with an equilibrium dissociation constant of 218 nM.	bind
22231	1	7117	6	13	NULL	NULL	NULL	NifX	GP		bind					FeMo-co	Chemical	finished			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_19_15968_s_239	11279153	2 The partial transfer of radio label from 55Fe-NifX to apodinitrogenase suggested that 55Fe-NifX is comprised of a mixture of either NifX bound to finished FeMo-co or to NifX bound to a FeMo-co precursor that is yet to be completed.	bind
22232	2	7117	6	13	NULL	NULL	NULL	NifX	GP		bind					FeMo-co precursor	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_19_15968_s_239	11279153	2 The partial transfer of radio label from 55Fe-NifX to apodinitrogenase suggested that 55Fe-NifX is comprised of a mixture of either NifX bound to finished FeMo-co or to NifX bound to a FeMo-co precursor that is yet to be completed.	bind
22233	3	7117	6	13	NULL	NULL	NULL	55Fe-NifX	GP		comprises of 					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_19_15968_s_239	11279153	2 The partial transfer of radio label from 55Fe-NifX to apodinitrogenase suggested that 55Fe-NifX is comprised of a mixture of either NifX bound to finished FeMo-co or to NifX bound to a FeMo-co precursor that is yet to be completed.	bind
22234	4	7117	6	13	NULL	NULL	NULL	55Fe-NifX	GP		comprises of					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_19_15968_s_239	11279153	2 The partial transfer of radio label from 55Fe-NifX to apodinitrogenase suggested that 55Fe-NifX is comprised of a mixture of either NifX bound to finished FeMo-co or to NifX bound to a FeMo-co precursor that is yet to be completed.	bind
26083	1	7117	7	NULL	NULL	0	NULL	NifX	NULL		bind	NULL				FeMo-co 	NULL	finished			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_19_15968_s_239	11279153	2 The partial transfer of radio label from 55Fe-NifX to apodinitrogenase suggested that 55Fe-NifX is comprised of a mixture of either NifX bound to finished FeMo-co or to NifX bound to a FeMo-co precursor that is yet to be completed.	bind
26084	2	7117	7	NULL	NULL	0	NULL	NifX	NULL		bind	NULL				FeMo-co precursor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_19_15968_s_239	11279153	2 The partial transfer of radio label from 55Fe-NifX to apodinitrogenase suggested that 55Fe-NifX is comprised of a mixture of either NifX bound to finished FeMo-co or to NifX bound to a FeMo-co precursor that is yet to be completed.	bind
26085	3	7117	7	NULL	NULL	0	NULL	55Fe-NifX	NULL		comprises of	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_19_15968_s_239	11279153	2 The partial transfer of radio label from 55Fe-NifX to apodinitrogenase suggested that 55Fe-NifX is comprised of a mixture of either NifX bound to finished FeMo-co or to NifX bound to a FeMo-co precursor that is yet to be completed.	bind
26086	4	7117	7	NULL	NULL	0	NULL	55Fe-NifX	NULL		comprises of	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_19_15968_s_239	11279153	2 The partial transfer of radio label from 55Fe-NifX to apodinitrogenase suggested that 55Fe-NifX is comprised of a mixture of either NifX bound to finished FeMo-co or to NifX bound to a FeMo-co precursor that is yet to be completed.	bind
22519	1	7118	6	13	NULL	NULL	NULL	heat shock			induces					hsp90beta gene	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_51_51143_s_200	14532285	2 The specificity of PKC-epsilon on heat shock-induced expression of the  hsp90beta gene is further supported by the fact that neither CA-PKC-alpha nor DN-PKC-alpha affected the promoter activity of the  hsp90beta gene in response to heat shock, suggesting that heat shock-induced expression of the  hsp90beta gene is regulated by a PKC-epsilon-dependent mechanism.	bind
22520	2	7118	6	13	NULL	NULL	NULL	statement 1	Process		is dependent on					PKC-epsilon	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_51_51143_s_200	14532285	2 The specificity of PKC-epsilon on heat shock-induced expression of the  hsp90beta gene is further supported by the fact that neither CA-PKC-alpha nor DN-PKC-alpha affected the promoter activity of the  hsp90beta gene in response to heat shock, suggesting that heat shock-induced expression of the  hsp90beta gene is regulated by a PKC-epsilon-dependent mechanism.	bind
22521	3	7118	6	13	NULL	NULL	NULL	CA-PKC-alpha	GP		does not affect					hsp90beta gene	GP	promoter activity of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_51_51143_s_200	14532285	2 The specificity of PKC-epsilon on heat shock-induced expression of the  hsp90beta gene is further supported by the fact that neither CA-PKC-alpha nor DN-PKC-alpha affected the promoter activity of the  hsp90beta gene in response to heat shock, suggesting that heat shock-induced expression of the  hsp90beta gene is regulated by a PKC-epsilon-dependent mechanism.	bind
22522	4	7118	6	13	NULL	NULL	NULL	DN-PKC-alpha	GP		does not affect					hsp90beta gene	GP	promoter activity of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_51_51143_s_200	14532285	2 The specificity of PKC-epsilon on heat shock-induced expression of the  hsp90beta gene is further supported by the fact that neither CA-PKC-alpha nor DN-PKC-alpha affected the promoter activity of the  hsp90beta gene in response to heat shock, suggesting that heat shock-induced expression of the  hsp90beta gene is regulated by a PKC-epsilon-dependent mechanism.	bind
53356	5	7118	6	13	NULL	NULL	NULL	statement 3	Process		occurs in response to					heat shock 					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_51_51143_s_200	14532285	2 The specificity of PKC-epsilon on heat shock-induced expression of the  hsp90beta gene is further supported by the fact that neither CA-PKC-alpha nor DN-PKC-alpha affected the promoter activity of the  hsp90beta gene in response to heat shock, suggesting that heat shock-induced expression of the  hsp90beta gene is regulated by a PKC-epsilon-dependent mechanism.	bind
53357	6	7118	6	13	NULL	NULL	NULL	statement 4	Process		occurs in response to					heat shock 					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_51_51143_s_200	14532285	2 The specificity of PKC-epsilon on heat shock-induced expression of the  hsp90beta gene is further supported by the fact that neither CA-PKC-alpha nor DN-PKC-alpha affected the promoter activity of the  hsp90beta gene in response to heat shock, suggesting that heat shock-induced expression of the  hsp90beta gene is regulated by a PKC-epsilon-dependent mechanism.	bind
26545	1	7118	7	10	NULL	0	NULL	CA-PKC-alpha	NULL		does not affect	NULL				hsp90beta	NULL	promoter activity of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_51_51143_s_200	14532285	2 The specificity of PKC-epsilon on heat shock-induced expression of the  hsp90beta gene is further supported by the fact that neither CA-PKC-alpha nor DN-PKC-alpha affected the promoter activity of the  hsp90beta gene in response to heat shock, suggesting that heat shock-induced expression of the  hsp90beta gene is regulated by a PKC-epsilon-dependent mechanism.	bind
26546	2	7118	7	10	NULL	0	NULL	DN-PKC-alpha	NULL		does not affect	NULL				hsp90beta	NULL	promoter activity of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_51_51143_s_200	14532285	2 The specificity of PKC-epsilon on heat shock-induced expression of the  hsp90beta gene is further supported by the fact that neither CA-PKC-alpha nor DN-PKC-alpha affected the promoter activity of the  hsp90beta gene in response to heat shock, suggesting that heat shock-induced expression of the  hsp90beta gene is regulated by a PKC-epsilon-dependent mechanism.	bind
26547	3	7118	7	NULL	NULL	0	NULL	statement 1	NULL		occurs in response to	NULL				heat shock 	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_51_51143_s_200	14532285	2 The specificity of PKC-epsilon on heat shock-induced expression of the  hsp90beta gene is further supported by the fact that neither CA-PKC-alpha nor DN-PKC-alpha affected the promoter activity of the  hsp90beta gene in response to heat shock, suggesting that heat shock-induced expression of the  hsp90beta gene is regulated by a PKC-epsilon-dependent mechanism.	bind
26548	4	7118	7	NULL	NULL	0	NULL	statement 2	NULL		occurs in response to	NULL				heat shock	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_51_51143_s_200	14532285	2 The specificity of PKC-epsilon on heat shock-induced expression of the  hsp90beta gene is further supported by the fact that neither CA-PKC-alpha nor DN-PKC-alpha affected the promoter activity of the  hsp90beta gene in response to heat shock, suggesting that heat shock-induced expression of the  hsp90beta gene is regulated by a PKC-epsilon-dependent mechanism.	bind
26549	5	7118	7	NULL	NULL	0	NULL	heat shock	NULL		induce	NULL				hsp90beta gene	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_51_51143_s_200	14532285	2 The specificity of PKC-epsilon on heat shock-induced expression of the  hsp90beta gene is further supported by the fact that neither CA-PKC-alpha nor DN-PKC-alpha affected the promoter activity of the  hsp90beta gene in response to heat shock, suggesting that heat shock-induced expression of the  hsp90beta gene is regulated by a PKC-epsilon-dependent mechanism.	bind
26550	6	7118	7	NULL	NULL	0	NULL	PKC-epsilon-dependent mechanism	NULL		regulates	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_51_51143_s_200	14532285	2 The specificity of PKC-epsilon on heat shock-induced expression of the  hsp90beta gene is further supported by the fact that neither CA-PKC-alpha nor DN-PKC-alpha affected the promoter activity of the  hsp90beta gene in response to heat shock, suggesting that heat shock-induced expression of the  hsp90beta gene is regulated by a PKC-epsilon-dependent mechanism.	bind
22235	1	7119	6	13	NULL	NULL	NULL	ATP	Chemical		bind								NBD		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29407_s_27	10893239	2 The structure of the ATP-binding subunit of the bacterial histidine transporter (HisP) provides a model for the binding of ATP to an NBD ( 9).	bind
26551	1	7119	7	NULL	NULL	0	NULL	ATP	NULL		bind	NULL					NULL		NBD		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29407_s_27	10893239	2 The structure of the ATP-binding subunit of the bacterial histidine transporter (HisP) provides a model for the binding of ATP to an NBD ( 9).	bind
22236	1	7120	6	13	NULL	NULL	NULL	CNX	GP		bind					glycoproteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_12_8623_s_172	11254652	2 The term "`lectin-like chaperone"` was originally introduced into the literature when the binding of CNX and CRT to glycoproteins was known to require specific oligosaccharide-dependent interactions, but the lectin activities for CNX and CRT remained to be demonstrated.	bind
22237	2	7120	6	13	NULL	NULL	NULL	CRT	GP		bind					glycoproteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_12_8623_s_172	11254652	2 The term "`lectin-like chaperone"` was originally introduced into the literature when the binding of CNX and CRT to glycoproteins was known to require specific oligosaccharide-dependent interactions, but the lectin activities for CNX and CRT remained to be demonstrated.	bind
22239	3	7120	6	13	NULL	NULL	NULL	statement 1	Process		require					oligosaccharide-dependent interactions	Process	specific			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_12_8623_s_172	11254652	2 The term "`lectin-like chaperone"` was originally introduced into the literature when the binding of CNX and CRT to glycoproteins was known to require specific oligosaccharide-dependent interactions, but the lectin activities for CNX and CRT remained to be demonstrated.	bind
22240	4	7120	6	13	NULL	NULL	NULL	statement 2	Process		require					oligosaccharide-dependent interactions	Process	specific			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_12_8623_s_172	11254652	2 The term "`lectin-like chaperone"` was originally introduced into the literature when the binding of CNX and CRT to glycoproteins was known to require specific oligosaccharide-dependent interactions, but the lectin activities for CNX and CRT remained to be demonstrated.	bind
26552	1	7120	7	NULL	NULL	0	NULL	CNX	NULL		bind	NULL				glycoproteins	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_12_8623_s_172	11254652	2 The term "`lectin-like chaperone"` was originally introduced into the literature when the binding of CNX and CRT to glycoproteins was known to require specific oligosaccharide-dependent interactions, but the lectin activities for CNX and CRT remained to be demonstrated.	bind
26553	2	7120	7	NULL	NULL	0	NULL	CRT	NULL		bind	NULL				glycoproteins	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_12_8623_s_172	11254652	2 The term "`lectin-like chaperone"` was originally introduced into the literature when the binding of CNX and CRT to glycoproteins was known to require specific oligosaccharide-dependent interactions, but the lectin activities for CNX and CRT remained to be demonstrated.	bind
26554	3	7120	7	NULL	NULL	0	NULL	statement 1	NULL		require	NULL				oligosaccharide-dependent interactions	NULL	specific			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_12_8623_s_172	11254652	2 The term "`lectin-like chaperone"` was originally introduced into the literature when the binding of CNX and CRT to glycoproteins was known to require specific oligosaccharide-dependent interactions, but the lectin activities for CNX and CRT remained to be demonstrated.	bind
26555	4	7120	7	NULL	NULL	0	NULL	statement 2	NULL		require	NULL				oligosaccharide-dependent interactions	NULL	specific			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_12_8623_s_172	11254652	2 The term "`lectin-like chaperone"` was originally introduced into the literature when the binding of CNX and CRT to glycoproteins was known to require specific oligosaccharide-dependent interactions, but the lectin activities for CNX and CRT remained to be demonstrated.	bind
22245	1	7121	6	13	NULL	NULL	NULL	Par6	GP	Drosophila	bind		directly			Patj	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_40_41557_s_169	15292221	2 There are also recent reports that the  Drosophila Par6 can bind directly to Patj (previously called Dlt) ( ), which is a binding partner for Pals1, and that Par6C can bind directly to the C terminus of Crb3 ( ), which is also a binding partner for Pals1.	bind
22249	2	7121	6	13	NULL	NULL	NULL	PatJ	GP		is 					Dlt	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_40_41557_s_169	15292221	2 There are also recent reports that the  Drosophila Par6 can bind directly to Patj (previously called Dlt) ( ), which is a binding partner for Pals1, and that Par6C can bind directly to the C terminus of Crb3 ( ), which is also a binding partner for Pals1.	bind
22254	3	7121	6	13	NULL	NULL	NULL	Patj	GP		bind					Pals1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_40_41557_s_169	15292221	2 There are also recent reports that the  Drosophila Par6 can bind directly to Patj (previously called Dlt) ( ), which is a binding partner for Pals1, and that Par6C can bind directly to the C terminus of Crb3 ( ), which is also a binding partner for Pals1.	bind
22259	4	7121	6	13	NULL	NULL	NULL	Par6C	GP		bind		directly			Crb3	GP		C terminus		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_40_41557_s_169	15292221	2 There are also recent reports that the  Drosophila Par6 can bind directly to Patj (previously called Dlt) ( ), which is a binding partner for Pals1, and that Par6C can bind directly to the C terminus of Crb3 ( ), which is also a binding partner for Pals1.	bind
22261	5	7121	6	13	NULL	NULL	NULL	Pals1	GP		bind					Crb3	GP		C terminus		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_40_41557_s_169	15292221	2 There are also recent reports that the  Drosophila Par6 can bind directly to Patj (previously called Dlt) ( ), which is a binding partner for Pals1, and that Par6C can bind directly to the C terminus of Crb3 ( ), which is also a binding partner for Pals1.	bind
26556	1	7121	7	NULL	NULL	0	NULL	Par6	NULL	Drosophila 	bind	NULL	directly			Patj	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_40_41557_s_169	15292221	2 There are also recent reports that the  Drosophila Par6 can bind directly to Patj (previously called Dlt) ( ), which is a binding partner for Pals1, and that Par6C can bind directly to the C terminus of Crb3 ( ), which is also a binding partner for Pals1.	bind
26557	2	7121	7	NULL	NULL	0	NULL	Patj	NULL		is	NULL				Dlt	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_40_41557_s_169	15292221	2 There are also recent reports that the  Drosophila Par6 can bind directly to Patj (previously called Dlt) ( ), which is a binding partner for Pals1, and that Par6C can bind directly to the C terminus of Crb3 ( ), which is also a binding partner for Pals1.	bind
26558	3	7121	7	NULL	NULL	0	NULL	Pals1	NULL		bind	NULL				Patj	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_40_41557_s_169	15292221	2 There are also recent reports that the  Drosophila Par6 can bind directly to Patj (previously called Dlt) ( ), which is a binding partner for Pals1, and that Par6C can bind directly to the C terminus of Crb3 ( ), which is also a binding partner for Pals1.	bind
26559	4	7121	7	NULL	NULL	0	NULL	Par6C	NULL		bind	NULL	directly			Crb3	NULL		C terminus		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_40_41557_s_169	15292221	2 There are also recent reports that the  Drosophila Par6 can bind directly to Patj (previously called Dlt) ( ), which is a binding partner for Pals1, and that Par6C can bind directly to the C terminus of Crb3 ( ), which is also a binding partner for Pals1.	bind
26560	5	7121	7	10	NULL	0	NULL	Pals1	NULL		bind	NULL				Crb3	NULL		C terminus		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_40_41557_s_169	15292221	2 There are also recent reports that the  Drosophila Par6 can bind directly to Patj (previously called Dlt) ( ), which is a binding partner for Pals1, and that Par6C can bind directly to the C terminus of Crb3 ( ), which is also a binding partner for Pals1.	bind
22269	1	7122	6	13	NULL	NULL	NULL	myosin phosphatase	GP		is a substrate for			regulatory myosin-binding subunit		PKG	GP				NULL	smooth muscle cell	NULL	NULL	NULL	NULL	gw60_circulationres_93_4_280_s_50	12933699	2 There are several specific physiological substrates for PKG in smooth muscle including the regulatory myosin-binding subunit of myosin phosphatase, 3 calcium-activated maxi K+ (BKCa) channels, 4 and IRAG (IP3 receptor associated cGMP kinase substrate).	bind
22271	2	7122	6	13	NULL	NULL	NULL	BKCa channels	GP		is a substrate for					PKG	GP				NULL	smooth muscle cell	NULL	NULL	NULL	NULL	gw60_circulationres_93_4_280_s_50	12933699	2 There are several specific physiological substrates for PKG in smooth muscle including the regulatory myosin-binding subunit of myosin phosphatase, 3 calcium-activated maxi K+ (BKCa) channels, 4 and IRAG (IP3 receptor associated cGMP kinase substrate).	bind
22272	3	7122	6	13	NULL	NULL	NULL	BKCa	GP		is					calcium-activated maxi K+ channels	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_4_280_s_50	12933699	2 There are several specific physiological substrates for PKG in smooth muscle including the regulatory myosin-binding subunit of myosin phosphatase, 3 calcium-activated maxi K+ (BKCa) channels, 4 and IRAG (IP3 receptor associated cGMP kinase substrate).	bind
22273	4	7122	6	13	NULL	NULL	NULL	IRAG	GP		is a substrate for					PKG	GP				NULL	smooth muscle cell	NULL	NULL	NULL	NULL	gw60_circulationres_93_4_280_s_50	12933699	2 There are several specific physiological substrates for PKG in smooth muscle including the regulatory myosin-binding subunit of myosin phosphatase, 3 calcium-activated maxi K+ (BKCa) channels, 4 and IRAG (IP3 receptor associated cGMP kinase substrate).	bind
22274	5	7122	6	13	NULL	NULL	NULL	IRAG	GP		is					IP3 receptor associated cGMP kinase substrate	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_4_280_s_50	12933699	2 There are several specific physiological substrates for PKG in smooth muscle including the regulatory myosin-binding subunit of myosin phosphatase, 3 calcium-activated maxi K+ (BKCa) channels, 4 and IRAG (IP3 receptor associated cGMP kinase substrate).	bind
37877	6	7122	6	13	NULL	NULL	NULL	IRAG	GP		is a type of					specific physiological substrate for PKG	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_4_280_s_50	12933699	2 There are several specific physiological substrates for PKG in smooth muscle including the regulatory myosin-binding subunit of myosin phosphatase, 3 calcium-activated maxi K+ (BKCa) channels, 4 and IRAG (IP3 receptor associated cGMP kinase substrate).	bind
37878	7	7122	6	13	NULL	NULL	NULL	myosin phosphatase	GP		is a type of					specific physiological substrate for PKG	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_4_280_s_50	12933699	2 There are several specific physiological substrates for PKG in smooth muscle including the regulatory myosin-binding subunit of myosin phosphatase, 3 calcium-activated maxi K+ (BKCa) channels, 4 and IRAG (IP3 receptor associated cGMP kinase substrate).	bind
37879	8	7122	6	13	NULL	NULL	NULL	BKCa channels	GP		is a type of					specific physiological substrate for PKG	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_4_280_s_50	12933699	2 There are several specific physiological substrates for PKG in smooth muscle including the regulatory myosin-binding subunit of myosin phosphatase, 3 calcium-activated maxi K+ (BKCa) channels, 4 and IRAG (IP3 receptor associated cGMP kinase substrate).	bind
26561	1	7122	7	NULL	NULL	0	NULL	myosin phosphatase	NULL		is a substrate of	NULL		regulatory myosin-binding subunit		PKG	NULL				NULL	smooth muscle	NULL	NULL	NULL	NULL	gw60_circulationres_93_4_280_s_50	12933699	2 There are several specific physiological substrates for PKG in smooth muscle including the regulatory myosin-binding subunit of myosin phosphatase, 3 calcium-activated maxi K+ (BKCa) channels, 4 and IRAG (IP3 receptor associated cGMP kinase substrate).	bind
26562	2	7122	7	NULL	NULL	0	NULL	BKCa	NULL		is a substrate of	NULL				PKG	NULL				NULL	smooth muscle	NULL	NULL	NULL	NULL	gw60_circulationres_93_4_280_s_50	12933699	2 There are several specific physiological substrates for PKG in smooth muscle including the regulatory myosin-binding subunit of myosin phosphatase, 3 calcium-activated maxi K+ (BKCa) channels, 4 and IRAG (IP3 receptor associated cGMP kinase substrate).	bind
26563	3	7122	7	NULL	NULL	0	NULL	IRAG	NULL		is a substrate of	NULL				PKG	NULL				NULL	smooth muscle	NULL	NULL	NULL	NULL	gw60_circulationres_93_4_280_s_50	12933699	2 There are several specific physiological substrates for PKG in smooth muscle including the regulatory myosin-binding subunit of myosin phosphatase, 3 calcium-activated maxi K+ (BKCa) channels, 4 and IRAG (IP3 receptor associated cGMP kinase substrate).	bind
26564	4	7122	7	NULL	NULL	0	NULL	BKCa	NULL		is	NULL				calcium-activated maxi K+ channels	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_93_4_280_s_50	12933699	2 There are several specific physiological substrates for PKG in smooth muscle including the regulatory myosin-binding subunit of myosin phosphatase, 3 calcium-activated maxi K+ (BKCa) channels, 4 and IRAG (IP3 receptor associated cGMP kinase substrate).	bind
26565	5	7122	7	NULL	NULL	0	NULL	IRAG	NULL		is	NULL				IP3 receptor associated cGMP kinase substrate	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_93_4_280_s_50	12933699	2 There are several specific physiological substrates for PKG in smooth muscle including the regulatory myosin-binding subunit of myosin phosphatase, 3 calcium-activated maxi K+ (BKCa) channels, 4 and IRAG (IP3 receptor associated cGMP kinase substrate).	bind
46446	6	7122	7	10	NULL	0	NULL	IRAG	NULL		is a type of	NULL				\tspecific physiological substrate for PKG	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_93_4_280_s_50	12933699	2 There are several specific physiological substrates for PKG in smooth muscle including the regulatory myosin-binding subunit of myosin phosphatase, 3 calcium-activated maxi K+ (BKCa) channels, 4 and IRAG (IP3 receptor associated cGMP kinase substrate).	bind
46447	7	7122	7	10	NULL	0	NULL	myosin phosphatase	NULL		is a type of	NULL				\tspecific physiological substrate for PKG	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_93_4_280_s_50	12933699	2 There are several specific physiological substrates for PKG in smooth muscle including the regulatory myosin-binding subunit of myosin phosphatase, 3 calcium-activated maxi K+ (BKCa) channels, 4 and IRAG (IP3 receptor associated cGMP kinase substrate).	bind
46448	8	7122	7	10	NULL	0	NULL	BKCa channels	NULL		is a type of	NULL				specific physiological substrate for PKG	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_93_4_280_s_50	12933699	2 There are several specific physiological substrates for PKG in smooth muscle including the regulatory myosin-binding subunit of myosin phosphatase, 3 calcium-activated maxi K+ (BKCa) channels, 4 and IRAG (IP3 receptor associated cGMP kinase substrate).	bind
22282	1	7124	6	13	NULL	NULL	NULL	target proteins	GP		do not contain								(K/R) XTQT motif		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_17_14059_s_249	11148209	2 Therefore, it is perhaps not surprising that DLC8 can bind a number of other target proteins, even though these proteins do not contain a (K/R) XTQT motif.	bind
22283	2	7124	6	13	NULL	NULL	NULL	DLC8	GP		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_17_14059_s_249	11148209	2 Therefore, it is perhaps not surprising that DLC8 can bind a number of other target proteins, even though these proteins do not contain a (K/R) XTQT motif.	bind
26567	1	7124	7	NULL	NULL	0	NULL	protein	NULL		does not contain	NULL					NULL		(K/R) XTQT motif		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_17_14059_s_249	11148209	2 Therefore, it is perhaps not surprising that DLC8 can bind a number of other target proteins, even though these proteins do not contain a (K/R) XTQT motif.	bind
26568	2	7124	7	NULL	NULL	0	NULL	DLC8	NULL		bind	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_17_14059_s_249	11148209	2 Therefore, it is perhaps not surprising that DLC8 can bind a number of other target proteins, even though these proteins do not contain a (K/R) XTQT motif.	bind
22289	1	7125	6	13	NULL	NULL	NULL	gentamicin	Chemical		bind					megalin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_1_618_s_163	11700326	2 Therefore, the antagonist is largely ineffective in blocking gentamicin binding to megalin.	bind
26569	1	7125	7	NULL	NULL	0	NULL	gentamicin	NULL		bind	NULL				megalin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_1_618_s_163	11700326	2 Therefore, the antagonist is largely ineffective in blocking gentamicin binding to megalin.	bind
22290	1	7126	6	13	NULL	NULL	NULL	histone H3	GP		bind					NF-I	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_3_1645_s_180	10636857	2 Therefore, the binding of histone H3 by NF-I may be the key step by which this transcription factor overcomes chromatin repression on both promoters and replication origins.	bind
22291	2	7126	6	13	NULL	NULL	NULL	NF-I 	GP		overcomes					chromatin	CellComponent	repression of		promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_3_1645_s_180	10636857	2 Therefore, the binding of histone H3 by NF-I may be the key step by which this transcription factor overcomes chromatin repression on both promoters and replication origins.	bind
22292	3	7126	6	13	NULL	NULL	NULL	NF-I	GP		overcomes					chromatin	CellComponent	repression of		replication origins	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_3_1645_s_180	10636857	2 Therefore, the binding of histone H3 by NF-I may be the key step by which this transcription factor overcomes chromatin repression on both promoters and replication origins.	bind
37406	4	7126	6	13	NULL	NULL	NULL	statement 1	Process		leads to		may			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_3_1645_s_180	10636857	2 Therefore, the binding of histone H3 by NF-I may be the key step by which this transcription factor overcomes chromatin repression on both promoters and replication origins.	bind
37407	5	7126	6	13	NULL	NULL	NULL	statement 1	Process		leads to		may			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_3_1645_s_180	10636857	2 Therefore, the binding of histone H3 by NF-I may be the key step by which this transcription factor overcomes chromatin repression on both promoters and replication origins.	bind
53358	6	7126	6	13	NULL	NULL	NULL	NF-I	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_3_1645_s_180	10636857	2 Therefore, the binding of histone H3 by NF-I may be the key step by which this transcription factor overcomes chromatin repression on both promoters and replication origins.	bind
26571	1	7126	7	NULL	NULL	0	NULL	NF-I	NULL		bind	NULL				histone H3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_3_1645_s_180	10636857	2 Therefore, the binding of histone H3 by NF-I may be the key step by which this transcription factor overcomes chromatin repression on both promoters and replication origins.	bind
26572	2	7126	7	10	NULL	0	NULL	NF-I	NULL		overcomes	NULL				chromatin	NULL	repression of		promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_3_1645_s_180	10636857	2 Therefore, the binding of histone H3 by NF-I may be the key step by which this transcription factor overcomes chromatin repression on both promoters and replication origins.	bind
26573	3	7126	7	10	NULL	0	NULL	NF-I	NULL		overcomes	NULL				chromatin	NULL	repression of		replication origin	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_3_1645_s_180	10636857	2 Therefore, the binding of histone H3 by NF-I may be the key step by which this transcription factor overcomes chromatin repression on both promoters and replication origins.	bind
26574	4	7126	7	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_3_1645_s_180	10636857	2 Therefore, the binding of histone H3 by NF-I may be the key step by which this transcription factor overcomes chromatin repression on both promoters and replication origins.	bind
26575	5	7126	7	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_3_1645_s_180	10636857	2 Therefore, the binding of histone H3 by NF-I may be the key step by which this transcription factor overcomes chromatin repression on both promoters and replication origins.	bind
53359	6	7126	7	10	NULL	0	NULL	NF-I	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_3_1645_s_180	10636857	2 Therefore, the binding of histone H3 by NF-I may be the key step by which this transcription factor overcomes chromatin repression on both promoters and replication origins.	bind
37408	1	7127	6	13	NULL	NULL	NULL	LARG-RhoA complex 	GP	changes in	reflect			P loop		GTPase	GP	plasticity of	active site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_45_47352_s_328	15331592	2 Therefore, the novel changes we observe in the P loop and the purine-binding pocket of the LARG-RhoA complex ( Fig. 5) probably reflect the natural plasticity of the GTPase active site when nucleotides are absent, rather than an active exchange mechanism exerted by the LARG DH domain.	bind
37409	2	7127	6	13	NULL	NULL	NULL	LARG-RhoA complex	GP	changes in	reflect			purine binding pocket		GTPase	GP	plasticity of	active site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_45_47352_s_328	15331592	2 Therefore, the novel changes we observe in the P loop and the purine-binding pocket of the LARG-RhoA complex ( Fig. 5) probably reflect the natural plasticity of the GTPase active site when nucleotides are absent, rather than an active exchange mechanism exerted by the LARG DH domain.	bind
37410	3	7127	6	13	NULL	NULL	NULL	statement 1	Process		occurs in absence of					nucleotides	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_45_47352_s_328	15331592	2 Therefore, the novel changes we observe in the P loop and the purine-binding pocket of the LARG-RhoA complex ( Fig. 5) probably reflect the natural plasticity of the GTPase active site when nucleotides are absent, rather than an active exchange mechanism exerted by the LARG DH domain.	bind
37411	4	7127	6	13	NULL	NULL	NULL	statement 2	Process		occurs in absence of					nucleotides	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_45_47352_s_328	15331592	2 Therefore, the novel changes we observe in the P loop and the purine-binding pocket of the LARG-RhoA complex ( Fig. 5) probably reflect the natural plasticity of the GTPase active site when nucleotides are absent, rather than an active exchange mechanism exerted by the LARG DH domain.	bind
26576	1	7127	7	NULL	NULL	0	NULL	LARG-RhoA complex	NULL	novel changes in	reflect	NULL		P loop		GTPase 	NULL	natural plasticity of	active site 		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_45_47352_s_328	15331592	2 Therefore, the novel changes we observe in the P loop and the purine-binding pocket of the LARG-RhoA complex ( Fig. 5) probably reflect the natural plasticity of the GTPase active site when nucleotides are absent, rather than an active exchange mechanism exerted by the LARG DH domain.	bind
26577	2	7127	7	NULL	NULL	0	NULL	 LARG-RhoA complex	NULL	novel changes in	reflect	NULL		 purine-binding pocket		GTPase 	NULL	natural plasticity of	active site 		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_45_47352_s_328	15331592	2 Therefore, the novel changes we observe in the P loop and the purine-binding pocket of the LARG-RhoA complex ( Fig. 5) probably reflect the natural plasticity of the GTPase active site when nucleotides are absent, rather than an active exchange mechanism exerted by the LARG DH domain.	bind
26578	3	7127	7	NULL	NULL	0	NULL	statement 1	NULL		in absence of	NULL				nucleotides	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_45_47352_s_328	15331592	2 Therefore, the novel changes we observe in the P loop and the purine-binding pocket of the LARG-RhoA complex ( Fig. 5) probably reflect the natural plasticity of the GTPase active site when nucleotides are absent, rather than an active exchange mechanism exerted by the LARG DH domain.	bind
26579	4	7127	7	NULL	NULL	0	NULL	statement 2	NULL		in absence of	NULL				nucleotides	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_45_47352_s_328	15331592	2 Therefore, the novel changes we observe in the P loop and the purine-binding pocket of the LARG-RhoA complex ( Fig. 5) probably reflect the natural plasticity of the GTPase active site when nucleotides are absent, rather than an active exchange mechanism exerted by the LARG DH domain.	bind
22296	1	7129	6	13	NULL	NULL	NULL				bind		directly	last seven amino acids of NR2 subunit		SAP90	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_35_21622_s_172	8702950	2 These data are similar to the recent findings, which suggested that the last seven amino acids of the NR2 subunit bind directly to SAP90 (Kornau  et al., 1995  ).	bind
26580	1	7129	7	NULL	NULL	0	NULL		NULL		bind	NULL	directly	last seven amino acids of  NR2 subunit		SAP90	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_35_21622_s_172	8702950	2 These data are similar to the recent findings, which suggested that the last seven amino acids of the NR2 subunit bind directly to SAP90 (Kornau  et al., 1995  ).	bind
22299	1	7130	6	13	NULL	NULL	NULL	CBP/p300	GP		bind					Py large T	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_36_33533_s_229	11438528	2 These findings indicate that CBP/p300 binding by Py large T is essential for virus growth.	bind
37417	2	7130	6	13	NULL	NULL	NULL	statement 1	Process		is essential for					virus growth	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_36_33533_s_229	11438528	2 These findings indicate that CBP/p300 binding by Py large T is essential for virus growth.	bind
26581	1	7130	7	NULL	NULL	0	NULL	Py large T	NULL		bind	NULL				CBP/p300	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_36_33533_s_229	11438528	2 These findings indicate that CBP/p300 binding by Py large T is essential for virus growth.	bind
26582	2	7130	7	NULL	NULL	0	NULL	statement 1	NULL		is essential for	NULL				virus growth	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_36_33533_s_229	11438528	2 These findings indicate that CBP/p300 binding by Py large T is essential for virus growth.	bind
22304	1	7131	6	13	NULL	NULL	NULL	heme	Chemical		bind					CBS	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_1_16_s_98	11042162	2 These findings indicate that under these conditions the heme groups that were bound to CBS had been completely released.	bind
26583	1	7131	7	NULL	NULL	0	NULL	heme groups	NULL		bind	NULL				CBS	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_16_s_98	11042162	2 These findings indicate that under these conditions the heme groups that were bound to CBS had been completely released.	bind
22312	1	7133	6	13	NULL	NULL	NULL	C/EBPdelta	GP		bind					HS3D	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31793_s_194	9395525	2 These results are now explained with the identification of C/EBPdelta as the nuclear protein binding to HS3D.	bind
37418	2	7133	6	13	NULL	NULL	NULL	C/EBPdelta	GP		is a type of					nuclear protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31793_s_194	9395525	2 These results are now explained with the identification of C/EBPdelta as the nuclear protein binding to HS3D.	bind
26584	1	7133	7	NULL	NULL	0	NULL	C/EBPdelta	NULL		bind	NULL				HS3D	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_50_31793_s_194	9395525	2 These results are now explained with the identification of C/EBPdelta as the nuclear protein binding to HS3D.	bind
26585	2	7133	7	NULL	NULL	0	NULL	C/EBPdelta	NULL		is a type of	NULL				nuclear protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_50_31793_s_194	9395525	2 These results are now explained with the identification of C/EBPdelta as the nuclear protein binding to HS3D.	bind
22523	1	7134	6	13	NULL	NULL	NULL	vinculin	GP		bind		may			beta-catenin	GP		vinculin binding site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_9078_s_202	9535896	2 These results raise the possibility that vinculin may bind beta-catenin with a lower affinity than does alpha-catenin or to a site on beta-catenin distinct from the alpha-catenin binding site that is sensitive to tyrosine phosphorylation.	bind
22524	2	7134	6	13	NULL	NULL	NULL	vinculin	GP		bind					beta-catenin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_9078_s_202	9535896	2 These results raise the possibility that vinculin may bind beta-catenin with a lower affinity than does alpha-catenin or to a site on beta-catenin distinct from the alpha-catenin binding site that is sensitive to tyrosine phosphorylation.	bind
22525	3	7134	6	13	NULL	NULL	NULL	statement 1	Process		lower affinity than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_9078_s_202	9535896	2 These results raise the possibility that vinculin may bind beta-catenin with a lower affinity than does alpha-catenin or to a site on beta-catenin distinct from the alpha-catenin binding site that is sensitive to tyrosine phosphorylation.	bind
22526	4	7134	6	13	NULL	NULL	NULL	beta-catenin	GP		is sensitive to			vinculin binding site		phosphorylation	Process		tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_9078_s_202	9535896	2 These results raise the possibility that vinculin may bind beta-catenin with a lower affinity than does alpha-catenin or to a site on beta-catenin distinct from the alpha-catenin binding site that is sensitive to tyrosine phosphorylation.	bind
26586	1	7134	7	NULL	NULL	0	NULL	vinculin	NULL		bind	NULL	may			beta-catenin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_9078_s_202	9535896	2 These results raise the possibility that vinculin may bind beta-catenin with a lower affinity than does alpha-catenin or to a site on beta-catenin distinct from the alpha-catenin binding site that is sensitive to tyrosine phosphorylation.	bind
26587	2	7134	7	NULL	NULL	0	NULL	vinculin	NULL		bind	NULL				alpha-catenin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_15_9078_s_202	9535896	2 These results raise the possibility that vinculin may bind beta-catenin with a lower affinity than does alpha-catenin or to a site on beta-catenin distinct from the alpha-catenin binding site that is sensitive to tyrosine phosphorylation.	bind
26588	3	7134	7	10	NULL	0	NULL	statement 1	NULL		lower affinity than	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_9078_s_202	9535896	2 These results raise the possibility that vinculin may bind beta-catenin with a lower affinity than does alpha-catenin or to a site on beta-catenin distinct from the alpha-catenin binding site that is sensitive to tyrosine phosphorylation.	bind
26589	4	7134	7	NULL	NULL	0	NULL	statement 1	NULL		is distinct from	NULL		binding site of		statement 2	NULL		binding site of		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_9078_s_202	9535896	2 These results raise the possibility that vinculin may bind beta-catenin with a lower affinity than does alpha-catenin or to a site on beta-catenin distinct from the alpha-catenin binding site that is sensitive to tyrosine phosphorylation.	bind
26590	5	7134	7	NULL	NULL	0	NULL	beta-catenin	NULL		is sensitive to	NULL		binding site		tyrosine phosphorylation	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_9078_s_202	9535896	2 These results raise the possibility that vinculin may bind beta-catenin with a lower affinity than does alpha-catenin or to a site on beta-catenin distinct from the alpha-catenin binding site that is sensitive to tyrosine phosphorylation.	bind
22316	1	7136	6	13	NULL	NULL	NULL	MT1 MMP	GP	active	bind			deltaTM 		heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_2_871_s_321	9422744	2 This domain appears to be responsible for the binding of active deltaTM MT1 MMP to heparin.	bind
26591	1	7136	7	NULL	NULL	0	NULL	 MT1 MMP	NULL	active	bind	NULL		deltaTM		heparin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_2_871_s_321	9422744	2 This domain appears to be responsible for the binding of active deltaTM MT1 MMP to heparin.	bind
22317	1	7137	6	13	NULL	NULL	NULL	RIP140	GP		bind		efficiently			AhR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_32_22155_s_205	10428779	2 This is also consistent with the fact that RIP140 can bind efficiently to AhR without its LBD (Fig.  2).	bind
22318	2	7137	6	13	NULL	NULL	NULL	statement 1	Process		occur in the absence of					RIP140	GP		LBD		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_32_22155_s_205	10428779	2 This is also consistent with the fact that RIP140 can bind efficiently to AhR without its LBD (Fig.  2).	bind
26592	1	7137	7	NULL	NULL	0	NULL	RIP140	NULL		bind	NULL	efficiently			AhR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_32_22155_s_205	10428779	2 This is also consistent with the fact that RIP140 can bind efficiently to AhR without its LBD (Fig.  2).	bind
26593	2	7137	7	NULL	NULL	0	NULL	statement 1	NULL		occur without	NULL				AhR	NULL		LBD		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_32_22155_s_205	10428779	2 This is also consistent with the fact that RIP140 can bind efficiently to AhR without its LBD (Fig.  2).	bind
22319	1	7138	6	13	NULL	NULL	NULL	gliotoxin	Chemical		bind		covalently						Cys-282		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_33_25202_s_164	10827185	2 This movement may be induced by covalent binding of gliotoxin to Cys-282.	bind
26594	1	7138	7	NULL	NULL	0	NULL	gliotoxin	NULL		bind	NULL	covalently				NULL		Cys-282		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_33_25202_s_164	10827185	2 This movement may be induced by covalent binding of gliotoxin to Cys-282.	bind
22320	1	7139	6	13	NULL	NULL	NULL	Sp1	GP		bind					E2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_41_25976_s_202	9325332	2 This observation and the immunoprecipitation/Western blot data presented above suggest a model in which Sp1 and Sp3 bind E2 and Puralpha binds E1 with Sp1 participating in protein-protein interactions with both Sp3 and Puralpha (Fig.  6).	bind
22321	2	7139	6	13	NULL	NULL	NULL	Sp3	GP		bind					E2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_41_25976_s_202	9325332	2 This observation and the immunoprecipitation/Western blot data presented above suggest a model in which Sp1 and Sp3 bind E2 and Puralpha binds E1 with Sp1 participating in protein-protein interactions with both Sp3 and Puralpha (Fig.  6).	bind
22322	3	7139	6	13	NULL	NULL	NULL	Puralpha	GP		bind					E1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_41_25976_s_202	9325332	2 This observation and the immunoprecipitation/Western blot data presented above suggest a model in which Sp1 and Sp3 bind E2 and Puralpha binds E1 with Sp1 participating in protein-protein interactions with both Sp3 and Puralpha (Fig.  6).	bind
22527	4	7139	6	13	NULL	NULL	NULL	Sp1	GP		interacts with					Sp3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_41_25976_s_202	9325332	2 This observation and the immunoprecipitation/Western blot data presented above suggest a model in which Sp1 and Sp3 bind E2 and Puralpha binds E1 with Sp1 participating in protein-protein interactions with both Sp3 and Puralpha (Fig.  6).	bind
22528	5	7139	6	13	NULL	NULL	NULL	Sp1	GP		interacts with					Puralpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_41_25976_s_202	9325332	2 This observation and the immunoprecipitation/Western blot data presented above suggest a model in which Sp1 and Sp3 bind E2 and Puralpha binds E1 with Sp1 participating in protein-protein interactions with both Sp3 and Puralpha (Fig.  6).	bind
26595	1	7139	7	NULL	NULL	0	NULL	Sp1	NULL		bind	NULL				E2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_41_25976_s_202	9325332	2 This observation and the immunoprecipitation/Western blot data presented above suggest a model in which Sp1 and Sp3 bind E2 and Puralpha binds E1 with Sp1 participating in protein-protein interactions with both Sp3 and Puralpha (Fig.  6).	bind
26596	2	7139	7	NULL	NULL	0	NULL	Sp3	NULL		bind	NULL				E2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_41_25976_s_202	9325332	2 This observation and the immunoprecipitation/Western blot data presented above suggest a model in which Sp1 and Sp3 bind E2 and Puralpha binds E1 with Sp1 participating in protein-protein interactions with both Sp3 and Puralpha (Fig.  6).	bind
26597	3	7139	7	NULL	NULL	0	NULL	Puralpha	NULL		binds	NULL				E1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_41_25976_s_202	9325332	2 This observation and the immunoprecipitation/Western blot data presented above suggest a model in which Sp1 and Sp3 bind E2 and Puralpha binds E1 with Sp1 participating in protein-protein interactions with both Sp3 and Puralpha (Fig.  6).	bind
26598	4	7139	7	NULL	NULL	0	NULL	 Sp1	NULL		bind	NULL				Sp3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_41_25976_s_202	9325332	2 This observation and the immunoprecipitation/Western blot data presented above suggest a model in which Sp1 and Sp3 bind E2 and Puralpha binds E1 with Sp1 participating in protein-protein interactions with both Sp3 and Puralpha (Fig.  6).	bind
26599	5	7139	7	NULL	NULL	0	NULL	Sp1	NULL		bind	NULL				Puralpha	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_41_25976_s_202	9325332	2 This observation and the immunoprecipitation/Western blot data presented above suggest a model in which Sp1 and Sp3 bind E2 and Puralpha binds E1 with Sp1 participating in protein-protein interactions with both Sp3 and Puralpha (Fig.  6).	bind
22326	1	7140	6	13	NULL	NULL	NULL	GEF-H1	GP		bind					Rho	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34954_s_174	9857026	2 This observation can be rationalized by the fact that GEF-H1 binds to Rho and Rac independently of their nucleotide binding status (Fig.  6) and therefore remains bound to RhoA-GTP even after the GDP/GTP exchange is accomplished.	bind
22327	2	7140	6	13	NULL	NULL	NULL	GEF-H1	GP		bind					Rac	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34954_s_174	9857026	2 This observation can be rationalized by the fact that GEF-H1 binds to Rho and Rac independently of their nucleotide binding status (Fig.  6) and therefore remains bound to RhoA-GTP even after the GDP/GTP exchange is accomplished.	bind
22329	3	7140	6	13	NULL	NULL	NULL	statement 1	Process		is independent of					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34954_s_174	9857026	2 This observation can be rationalized by the fact that GEF-H1 binds to Rho and Rac independently of their nucleotide binding status (Fig.  6) and therefore remains bound to RhoA-GTP even after the GDP/GTP exchange is accomplished.	bind
22331	4	7140	6	13	NULL	NULL	NULL	statement 2	Process		is independent of					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34954_s_174	9857026	2 This observation can be rationalized by the fact that GEF-H1 binds to Rho and Rac independently of their nucleotide binding status (Fig.  6) and therefore remains bound to RhoA-GTP even after the GDP/GTP exchange is accomplished.	bind
22333	5	7140	6	13	NULL	NULL	NULL	GEF-H1	GP		bind					RhoA-GTP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34954_s_174	9857026	2 This observation can be rationalized by the fact that GEF-H1 binds to Rho and Rac independently of their nucleotide binding status (Fig.  6) and therefore remains bound to RhoA-GTP even after the GDP/GTP exchange is accomplished.	bind
22334	6	7140	6	13	NULL	NULL	NULL	statement 5	Process		occurs after					GDP/GTP 	Process	exchange of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34954_s_174	9857026	2 This observation can be rationalized by the fact that GEF-H1 binds to Rho and Rac independently of their nucleotide binding status (Fig.  6) and therefore remains bound to RhoA-GTP even after the GDP/GTP exchange is accomplished.	bind
55796	7	7140	6	13	NULL	NULL	NULL	Rho	GP		bind					nucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34954_s_174	9857026	2 This observation can be rationalized by the fact that GEF-H1 binds to Rho and Rac independently of their nucleotide binding status (Fig.  6) and therefore remains bound to RhoA-GTP even after the GDP/GTP exchange is accomplished.	bind
55797	8	7140	6	13	NULL	NULL	NULL	Rac	GP		bind					nucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34954_s_174	9857026	2 This observation can be rationalized by the fact that GEF-H1 binds to Rho and Rac independently of their nucleotide binding status (Fig.  6) and therefore remains bound to RhoA-GTP even after the GDP/GTP exchange is accomplished.	bind
26600	3	7140	7	NULL	NULL	0	NULL	GEF-H1			bind					Rho					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34954_s_174	9857026	2 This observation can be rationalized by the fact that GEF-H1 binds to Rho and Rac independently of their nucleotide binding status (Fig.  6) and therefore remains bound to RhoA-GTP even after the GDP/GTP exchange is accomplished.	bind
26601	4	7140	7	NULL	NULL	0	NULL	GEF-H1			bind					Rac					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34954_s_174	9857026	2 This observation can be rationalized by the fact that GEF-H1 binds to Rho and Rac independently of their nucleotide binding status (Fig.  6) and therefore remains bound to RhoA-GTP even after the GDP/GTP exchange is accomplished.	bind
26602	4	7140	7	NULL	NULL	0	NULL	statement 3			is independent of					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34954_s_174	9857026	2 This observation can be rationalized by the fact that GEF-H1 binds to Rho and Rac independently of their nucleotide binding status (Fig.  6) and therefore remains bound to RhoA-GTP even after the GDP/GTP exchange is accomplished.	bind
26603	6	7140	7	NULL	NULL	0	NULL	statement 4			is independent of					statement 2					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34954_s_174	9857026	2 This observation can be rationalized by the fact that GEF-H1 binds to Rho and Rac independently of their nucleotide binding status (Fig.  6) and therefore remains bound to RhoA-GTP even after the GDP/GTP exchange is accomplished.	bind
26604	7	7140	7	NULL	NULL	0	NULL	GEF-H1			bind					RhoA-GTP					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34954_s_174	9857026	2 This observation can be rationalized by the fact that GEF-H1 binds to Rho and Rac independently of their nucleotide binding status (Fig.  6) and therefore remains bound to RhoA-GTP even after the GDP/GTP exchange is accomplished.	bind
26606	8	7140	7	NULL	NULL	0	NULL	statement 7			occurs after					GDP/GTP		exchange of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34954_s_174	9857026	2 This observation can be rationalized by the fact that GEF-H1 binds to Rho and Rac independently of their nucleotide binding status (Fig.  6) and therefore remains bound to RhoA-GTP even after the GDP/GTP exchange is accomplished.	bind
54626	1	7140	7	NULL	NULL	0	NULL	Rho			bind					nucleotide					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_52_34954_s_174	9857026	2 This observation can be rationalized by the fact that GEF-H1 binds to Rho and Rac independently of their nucleotide binding status (Fig.  6) and therefore remains bound to RhoA-GTP even after the GDP/GTP exchange is accomplished.	bind
54627	2	7140	7	NULL	NULL	0	NULL	Rac			bind					nucleotide					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34954_s_174	9857026	2 This observation can be rationalized by the fact that GEF-H1 binds to Rho and Rac independently of their nucleotide binding status (Fig.  6) and therefore remains bound to RhoA-GTP even after the GDP/GTP exchange is accomplished.	bind
22529	1	7141	6	13	NULL	NULL	NULL	HSP70	GP		activates					TLR2 transfected cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_15107_s_186	11842086	2 This question needs to be addressed by analyzing whether inhibition of endocytosis differentially affects HSP70-driven activation of TLR2-transfected  versus TLR4 plus MD-2-transfected cells.	bind
22530	2	7141	6	13	NULL	NULL	NULL	HSP70	GP		activates					TLR4 plus MD-2-transfected cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_15107_s_186	11842086	2 This question needs to be addressed by analyzing whether inhibition of endocytosis differentially affects HSP70-driven activation of TLR2-transfected  versus TLR4 plus MD-2-transfected cells.	bind
26628	1	7141	7	NULL	NULL	0	NULL	HSP70	NULL		activates	NULL				TLR2-transfected cells	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_17_15107_s_186	11842086	2 This question needs to be addressed by analyzing whether inhibition of endocytosis differentially affects HSP70-driven activation of TLR2-transfected  versus TLR4 plus MD-2-transfected cells.	bind
26629	2	7141	7	NULL	NULL	0	NULL	HSP70	NULL		activates	NULL				TLR4 plus MD-2-transfected cells	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_15107_s_186	11842086	2 This question needs to be addressed by analyzing whether inhibition of endocytosis differentially affects HSP70-driven activation of TLR2-transfected  versus TLR4 plus MD-2-transfected cells.	bind
22373	1	7142	6	13	NULL	NULL	NULL	HDL	GP		bind		might;;directly			CD36	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_41_26338_s_124	9756864	2 This raised the possibility that, as is the case with the other well characterized class B scavenger receptor SR-BI, HDL might bind directly to CD36.	bind
22374	2	7142	6	13	NULL	NULL	NULL	SR-BI	GP		is a type of					class B scavenger receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_41_26338_s_124	9756864	2 This raised the possibility that, as is the case with the other well characterized class B scavenger receptor SR-BI, HDL might bind directly to CD36.	bind
37421	3	7142	6	13	NULL	NULL	NULL	SR-BI	GP		bind		directly			CD36	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_41_26338_s_124	9756864	2 This raised the possibility that, as is the case with the other well characterized class B scavenger receptor SR-BI, HDL might bind directly to CD36.	bind
26630	1	7142	7	NULL	NULL	0	NULL	SR-BI	NULL		bind	NULL	directly			CD36	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_41_26338_s_124	9756864	2 This raised the possibility that, as is the case with the other well characterized class B scavenger receptor SR-BI, HDL might bind directly to CD36.	bind
26631	2	7142	7	NULL	NULL	0	NULL	HDL	NULL		bind	NULL	might;;directly			CD36	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_41_26338_s_124	9756864	2 This raised the possibility that, as is the case with the other well characterized class B scavenger receptor SR-BI, HDL might bind directly to CD36.	bind
26632	3	7142	7	NULL	NULL	0	NULL	SR-BI	NULL		is a type of	NULL				class B scavenger receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_41_26338_s_124	9756864	2 This raised the possibility that, as is the case with the other well characterized class B scavenger receptor SR-BI, HDL might bind directly to CD36.	bind
22375	1	7143	6	13	NULL	NULL	NULL	CDH1 gene	GP		encode 				exon 6	NLS	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_14_12530_s_148	12560341	2 This raises the possibility that exons 6 and 7 of the  CDH1 gene could encode an NLS.	bind
22376	2	7143	6	13	NULL	NULL	NULL	CDH1 gene	GP		encode				exon 7	NLS	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_14_12530_s_148	12560341	2 This raises the possibility that exons 6 and 7 of the  CDH1 gene could encode an NLS.	bind
26633	1	7143	7	NULL	NULL	0	NULL	CDH1 gene	NULL		encode	NULL			exon 6	NLS	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_14_12530_s_148	12560341	2 This raises the possibility that exons 6 and 7 of the  CDH1 gene could encode an NLS.	bind
26634	2	7143	7	NULL	NULL	0	NULL	CDH1 gene	NULL		encode	NULL			exon 7	NLS	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_14_12530_s_148	12560341	2 This raises the possibility that exons 6 and 7 of the  CDH1 gene could encode an NLS.	bind
22377	1	7144	6	13	NULL	NULL	NULL	Cl	Chemical	oxygen-linked	bind					Hb	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39048_s_166	10984477	2 This Root effect fish Hb is fully responsive to phosphates but has a blocked alpha-N terminus and thus lacks one of the residues of importance in oxygen-linked Cl  binding to human Hb ( 52).	bind
22378	2	7144	6	13	NULL	NULL	NULL	Hb	GP	fish	is responsive to		fully			phosphates	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39048_s_166	10984477	2 This Root effect fish Hb is fully responsive to phosphates but has a blocked alpha-N terminus and thus lacks one of the residues of importance in oxygen-linked Cl  binding to human Hb ( 52).	bind
22379	3	7144	6	13	NULL	NULL	NULL	Hb	GP	fish	contains							blocked	alpha-N terminus		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39048_s_166	10984477	2 This Root effect fish Hb is fully responsive to phosphates but has a blocked alpha-N terminus and thus lacks one of the residues of importance in oxygen-linked Cl  binding to human Hb ( 52).	bind
26635	1	7144	7	NULL	NULL	0	NULL	 Cl	NULL	oxygen-linked	bind	NULL				Hb	NULL	human			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_50_39048_s_166	10984477	2 This Root effect fish Hb is fully responsive to phosphates but has a blocked alpha-N terminus and thus lacks one of the residues of importance in oxygen-linked Cl  binding to human Hb ( 52).	bind
26636	2	7144	7	10	NULL	0	NULL	Hb	NULL	fish	is responsive to	NULL	fully			phosphates	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39048_s_166	10984477	2 This Root effect fish Hb is fully responsive to phosphates but has a blocked alpha-N terminus and thus lacks one of the residues of importance in oxygen-linked Cl  binding to human Hb ( 52).	bind
26637	3	7144	7	10	NULL	0	NULL	Hb	NULL	fish	contains	NULL					NULL	blocked	alpha-N terminus		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39048_s_166	10984477	2 This Root effect fish Hb is fully responsive to phosphates but has a blocked alpha-N terminus and thus lacks one of the residues of importance in oxygen-linked Cl  binding to human Hb ( 52).	bind
26638	4	7144	7	NULL	NULL	0	NULL	Hb	NULL	fish	lacks	NULL				statement 1	NULL	residues for			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_50_39048_s_166	10984477	2 This Root effect fish Hb is fully responsive to phosphates but has a blocked alpha-N terminus and thus lacks one of the residues of importance in oxygen-linked Cl  binding to human Hb ( 52).	bind
22380	1	7145	6	13	NULL	NULL	NULL	IRS-1	GP		bind		might	Tyr- X-X-Met motifs		PI 3 kinase	GP				NULL	insulin sensitive tissues	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_45_28677_s_123	8910502	2 Thus in insulin-sensitive tissues, Tyr- X-X-Met motifs other than Tyr-460, -608, -939, and -987 of IRS-1 might bind and activate PI 3-kinase in response to insulin.	bind
22381	2	7145	6	13	NULL	NULL	NULL	statement 1	Process		activate		might			PI 3 kinase	GP				NULL	insulin sensitive tissues	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_45_28677_s_123	8910502	2 Thus in insulin-sensitive tissues, Tyr- X-X-Met motifs other than Tyr-460, -608, -939, and -987 of IRS-1 might bind and activate PI 3-kinase in response to insulin.	bind
22382	3	7145	6	13	NULL	NULL	NULL	statement 2	Process		occurs in response to					insulin	GP				NULL	insulin sensitive tissues	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_45_28677_s_123	8910502	2 Thus in insulin-sensitive tissues, Tyr- X-X-Met motifs other than Tyr-460, -608, -939, and -987 of IRS-1 might bind and activate PI 3-kinase in response to insulin.	bind
22383	4	7145	6	13	NULL	NULL	NULL	IRS-1	GP		does not bind			Tyr-460		PI 3 kinase	GP				NULL	insulin sensitive tissues	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_45_28677_s_123	8910502	2 Thus in insulin-sensitive tissues, Tyr- X-X-Met motifs other than Tyr-460, -608, -939, and -987 of IRS-1 might bind and activate PI 3-kinase in response to insulin.	bind
22384	5	7145	6	13	NULL	NULL	NULL	IRS-1	GP		does not bind			Tyr-608		PI 3 kinase	GP				NULL	insulin sensitive tissues	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_45_28677_s_123	8910502	2 Thus in insulin-sensitive tissues, Tyr- X-X-Met motifs other than Tyr-460, -608, -939, and -987 of IRS-1 might bind and activate PI 3-kinase in response to insulin.	bind
22385	6	7145	6	13	NULL	NULL	NULL	IRS-1	GP		does not bind			Tyr-939		PI 3 kinase	GP				NULL	insulin sensitive tissues	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_45_28677_s_123	8910502	2 Thus in insulin-sensitive tissues, Tyr- X-X-Met motifs other than Tyr-460, -608, -939, and -987 of IRS-1 might bind and activate PI 3-kinase in response to insulin.	bind
22386	7	7145	6	13	NULL	NULL	NULL	IRS-1	GP		does not bind			Tyr-987		PI 3 kinase	GP				NULL	insulin sensitive tissues	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_45_28677_s_123	8910502	2 Thus in insulin-sensitive tissues, Tyr- X-X-Met motifs other than Tyr-460, -608, -939, and -987 of IRS-1 might bind and activate PI 3-kinase in response to insulin.	bind
26639	1	7145	7	10	NULL	0	NULL	IRS-1	NULL		bind	NULL	might	Tyr- X-X-Met motif		PI 3-kinase	NULL				NULL	insulin-sensitive tissues	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_45_28677_s_123	8910502	2 Thus in insulin-sensitive tissues, Tyr- X-X-Met motifs other than Tyr-460, -608, -939, and -987 of IRS-1 might bind and activate PI 3-kinase in response to insulin.	bind
26646	2	7145	7	10	NULL	0	NULL	statement 1	NULL		activate	NULL	might			PI 3-kinase	NULL				NULL	insulin-sensitive tissues	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_45_28677_s_123	8910502	2 Thus in insulin-sensitive tissues, Tyr- X-X-Met motifs other than Tyr-460, -608, -939, and -987 of IRS-1 might bind and activate PI 3-kinase in response to insulin.	bind
26650	3	7145	7	NULL	NULL	0	NULL	IRS-1	NULL		does not bind	NULL		 Tyr-460		PI 3-kinase	NULL				NULL	insulin-sensitive tissues	0	NULL	NULL	NULL	gw60_jbiolchem_271_45_28677_s_123	8910502	2 Thus in insulin-sensitive tissues, Tyr- X-X-Met motifs other than Tyr-460, -608, -939, and -987 of IRS-1 might bind and activate PI 3-kinase in response to insulin.	bind
26663	4	7145	7	NULL	NULL	0	NULL	 IRS-1 	NULL		does not bind	NULL		Tyr-608		PI 3-kinase	NULL				NULL	 insulin-sensitive tissues	0	NULL	NULL	NULL	gw60_jbiolchem_271_45_28677_s_123	8910502	2 Thus in insulin-sensitive tissues, Tyr- X-X-Met motifs other than Tyr-460, -608, -939, and -987 of IRS-1 might bind and activate PI 3-kinase in response to insulin.	bind
26669	5	7145	7	NULL	NULL	0	NULL	IRS-1	NULL		does not bind	NULL		Tyr-939		PI 3-kinase	NULL				NULL	insulin-sensitive tissues	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_45_28677_s_123	8910502	2 Thus in insulin-sensitive tissues, Tyr- X-X-Met motifs other than Tyr-460, -608, -939, and -987 of IRS-1 might bind and activate PI 3-kinase in response to insulin.	bind
26671	6	7145	7	NULL	NULL	0	NULL	IRS-1	NULL		does not bind	NULL		Tyr-987		PI 3-kinase	NULL				NULL	insulin-sensitive tissues	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_45_28677_s_123	8910502	2 Thus in insulin-sensitive tissues, Tyr- X-X-Met motifs other than Tyr-460, -608, -939, and -987 of IRS-1 might bind and activate PI 3-kinase in response to insulin.	bind
26673	7	7145	7	NULL	NULL	0	NULL	statement 2	NULL		occurs in response to	NULL				insulin	NULL				NULL	insulin-sensitive tissues	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_45_28677_s_123	8910502	2 Thus in insulin-sensitive tissues, Tyr- X-X-Met motifs other than Tyr-460, -608, -939, and -987 of IRS-1 might bind and activate PI 3-kinase in response to insulin.	bind
22387	1	7146	6	13	NULL	NULL	NULL	Bud6	GP		stimulates					formin	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_30_28023_s_276	15923184	2 Thus, all detectable binding and stimulation of formin activity by Bud6 is specific to Bni1 and not Bnr1.	bind
22388	2	7146	6	13	NULL	NULL	NULL	statement 1	Process		is specific to					Bni1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_30_28023_s_276	15923184	2 Thus, all detectable binding and stimulation of formin activity by Bud6 is specific to Bni1 and not Bnr1.	bind
22389	3	7146	6	13	NULL	NULL	NULL	statement 1	Process		is not specific to					Bnr1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_30_28023_s_276	15923184	2 Thus, all detectable binding and stimulation of formin activity by Bud6 is specific to Bni1 and not Bnr1.	bind
26686	1	7146	7	NULL	NULL	0	NULL	Bud6	NULL		stimulates	NULL				formin	NULL	activity of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_30_28023_s_276	15923184	2 Thus, all detectable binding and stimulation of formin activity by Bud6 is specific to Bni1 and not Bnr1.	bind
26687	2	7146	7	10	NULL	0	NULL	statement 1			is specific to					Bni1					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_30_28023_s_276	15923184	2 Thus, all detectable binding and stimulation of formin activity by Bud6 is specific to Bni1 and not Bnr1.	bind
26688	3	7146	7	NULL	NULL	0	NULL	statement 1	NULL		is not specific to	NULL				Bnr1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_30_28023_s_276	15923184	2 Thus, all detectable binding and stimulation of formin activity by Bud6 is specific to Bni1 and not Bnr1.	bind
22390	1	7147	6	13	NULL	NULL	NULL	HNF4	GP		bind								HNF4 binding site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_30_19339_s_41	9668124	2 Thus, although some of our results agreed with that reported by Waltz  et al. ( 17), we could not explain tissue-specific expression of MSP mRNA simply by the binding of HNF-4 to the previously reported HNF-4-binding site.	bind
22391	2	7147	6	13	NULL	NULL	NULL	MSP mRNA	NucleicAcid		is specific to					tissue	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_30_19339_s_41	9668124	2 Thus, although some of our results agreed with that reported by Waltz  et al. ( 17), we could not explain tissue-specific expression of MSP mRNA simply by the binding of HNF-4 to the previously reported HNF-4-binding site.	bind
26689	1	7147	7	NULL	NULL	0	NULL	HNF-4 	NULL		bind	NULL					NULL		HNF-4-binding site		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_30_19339_s_41	9668124	2 Thus, although some of our results agreed with that reported by Waltz  et al. ( 17), we could not explain tissue-specific expression of MSP mRNA simply by the binding of HNF-4 to the previously reported HNF-4-binding site.	bind
37491	2	7147	7	NULL	NULL	0	NULL	MSP mRNA	NULL		is specific to	NULL				tissue	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_30_19339_s_41	9668124	2 Thus, although some of our results agreed with that reported by Waltz  et al. ( 17), we could not explain tissue-specific expression of MSP mRNA simply by the binding of HNF-4 to the previously reported HNF-4-binding site.	bind
22392	1	7148	6	13	NULL	NULL	NULL	RecA protein	GP		bind		directly			dsDNA substrate	NucleicAcid	linear			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_17_11063_s_132	9111000	2 Thus, any effect of direct RecA protein binding to the linear dsDNA substrate (prior to its involvement in DNA strand exchange) can be neglected on the time scale used in these reactions.	bind
22393	2	7148	6	13	NULL	NULL	NULL	RecA protein	GP		is involved in					DNA strand exchange	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_17_11063_s_132	9111000	2 Thus, any effect of direct RecA protein binding to the linear dsDNA substrate (prior to its involvement in DNA strand exchange) can be neglected on the time scale used in these reactions.	bind
26690	1	7148	7	NULL	NULL	0	NULL	RecA protein	NULL		bind	NULL	directly			dsDNA substrate	NULL	linear			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_17_11063_s_132	9111000	2 Thus, any effect of direct RecA protein binding to the linear dsDNA substrate (prior to its involvement in DNA strand exchange) can be neglected on the time scale used in these reactions.	bind
37492	2	7148	7	NULL	NULL	0	NULL	RecA protein	NULL		is involved in	NULL				DNA strand exchange	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_17_11063_s_132	9111000	2 Thus, any effect of direct RecA protein binding to the linear dsDNA substrate (prior to its involvement in DNA strand exchange) can be neglected on the time scale used in these reactions.	bind
22394	1	7149	6	13	NULL	NULL	NULL	MEKK1	GP		bind		stably			GCK	GP	free	CTD		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_35_22681_s_205	9712898	2 Thus, MEKK1 binds most stably to the free GCK-CTD; binding of GCK to full-length GCK, while detectable, is less avid, and kinase-inactive GCK binds MEKK1 less stably than does wild type GCK.	bind
22395	2	7149	6	13	NULL	NULL	NULL	GCK	GP		bind					GCK	GP	full length			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_35_22681_s_205	9712898	2 Thus, MEKK1 binds most stably to the free GCK-CTD; binding of GCK to full-length GCK, while detectable, is less avid, and kinase-inactive GCK binds MEKK1 less stably than does wild type GCK.	bind
22396	3	7149	6	13	NULL	NULL	NULL	GCK	GP	kinase inactive	bind					MEKK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_35_22681_s_205	9712898	2 Thus, MEKK1 binds most stably to the free GCK-CTD; binding of GCK to full-length GCK, while detectable, is less avid, and kinase-inactive GCK binds MEKK1 less stably than does wild type GCK.	bind
22397	4	7149	6	13	NULL	NULL	NULL	statement 3	Process		is less stable than					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_35_22681_s_205	9712898	2 Thus, MEKK1 binds most stably to the free GCK-CTD; binding of GCK to full-length GCK, while detectable, is less avid, and kinase-inactive GCK binds MEKK1 less stably than does wild type GCK.	bind
37424	5	7149	6	13	NULL	NULL	NULL	GCK	GP	wild type	bind					MEKK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_35_22681_s_205	9712898	2 Thus, MEKK1 binds most stably to the free GCK-CTD; binding of GCK to full-length GCK, while detectable, is less avid, and kinase-inactive GCK binds MEKK1 less stably than does wild type GCK.	bind
26691	1	7149	7	NULL	NULL	0	NULL	MEKK1	NULL		bind	NULL	stably			GCK	NULL	free	CTD		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_35_22681_s_205	9712898	2 Thus, MEKK1 binds most stably to the free GCK-CTD; binding of GCK to full-length GCK, while detectable, is less avid, and kinase-inactive GCK binds MEKK1 less stably than does wild type GCK.	bind
26692	2	7149	7	NULL	NULL	0	NULL	GCK 	NULL		bind	NULL				GCK	NULL	full-length			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_35_22681_s_205	9712898	2 Thus, MEKK1 binds most stably to the free GCK-CTD; binding of GCK to full-length GCK, while detectable, is less avid, and kinase-inactive GCK binds MEKK1 less stably than does wild type GCK.	bind
26693	3	7149	7	NULL	NULL	0	NULL	GCK	NULL	kinase-inactive	binds	NULL				MEKK1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_35_22681_s_205	9712898	2 Thus, MEKK1 binds most stably to the free GCK-CTD; binding of GCK to full-length GCK, while detectable, is less avid, and kinase-inactive GCK binds MEKK1 less stably than does wild type GCK.	bind
26694	4	7149	7	NULL	NULL	0	NULL	GCK	NULL	wild type	binds	NULL				MEKK1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_35_22681_s_205	9712898	2 Thus, MEKK1 binds most stably to the free GCK-CTD; binding of GCK to full-length GCK, while detectable, is less avid, and kinase-inactive GCK binds MEKK1 less stably than does wild type GCK.	bind
26695	5	7149	7	10	NULL	0	NULL	statement 3	NULL		 less stable than	NULL				statement 4	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_35_22681_s_205	9712898	2 Thus, MEKK1 binds most stably to the free GCK-CTD; binding of GCK to full-length GCK, while detectable, is less avid, and kinase-inactive GCK binds MEKK1 less stably than does wild type GCK.	bind
22398	1	7150	6	13	NULL	NULL	NULL	decorin	GP		bind					collagen type I	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_29_18404_s_132	9218483	2 Thus, primarily ionic interactions appear to be responsible for the binding between decorin and type I collagen.	bind
22399	2	7150	6	13	NULL	NULL	NULL	ionic interactions	Process		is responsible for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_29_18404_s_132	9218483	2 Thus, primarily ionic interactions appear to be responsible for the binding between decorin and type I collagen.	bind
26696	1	7150	7	NULL	NULL	0	NULL	decorin	NULL		bind	NULL				type I collagen	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_29_18404_s_132	9218483	2 Thus, primarily ionic interactions appear to be responsible for the binding between decorin and type I collagen.	bind
26697	2	7150	7	NULL	NULL	0	NULL	ionic interactions	NULL		is responsible for	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_29_18404_s_132	9218483	2 Thus, primarily ionic interactions appear to be responsible for the binding between decorin and type I collagen.	bind
22400	1	7151	6	13	NULL	NULL	NULL	Tat	GP		interacts with					microtubules	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_46_48197_s_275	15331610	2 Thus, the difference in the speed of apoptosis could be due to the efficiency with which Tat interacts with microtubules, and the  in vitro data presented here show that Ug05RP bound to tubulin with a higher affinity compared with Ug11LTS.	bind
22401	2	7151	6	13	NULL	NULL	NULL	Ug05RP	GP		bind					tubulin	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_46_48197_s_275	15331610	2 Thus, the difference in the speed of apoptosis could be due to the efficiency with which Tat interacts with microtubules, and the  in vitro data presented here show that Ug05RP bound to tubulin with a higher affinity compared with Ug11LTS.	bind
22402	3	7151	6	13	NULL	NULL	NULL	Ug11LTS	GP		bind					tubulin	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_46_48197_s_275	15331610	2 Thus, the difference in the speed of apoptosis could be due to the efficiency with which Tat interacts with microtubules, and the  in vitro data presented here show that Ug05RP bound to tubulin with a higher affinity compared with Ug11LTS.	bind
22403	4	7151	6	13	NULL	NULL	NULL	statement 2	Process		is higher than					statement 3	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_46_48197_s_275	15331610	2 Thus, the difference in the speed of apoptosis could be due to the efficiency with which Tat interacts with microtubules, and the  in vitro data presented here show that Ug05RP bound to tubulin with a higher affinity compared with Ug11LTS.	bind
22404	5	7151	6	13	NULL	NULL	NULL	statement 1	Process	efficiency of	change					apoptosis	Process	speed of 			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_46_48197_s_275	15331610	2 Thus, the difference in the speed of apoptosis could be due to the efficiency with which Tat interacts with microtubules, and the  in vitro data presented here show that Ug05RP bound to tubulin with a higher affinity compared with Ug11LTS.	bind
26698	1	7151	7	NULL	NULL	0	NULL	Tat	NULL		interacts with	NULL				microtubules	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_46_48197_s_275	15331610	2 Thus, the difference in the speed of apoptosis could be due to the efficiency with which Tat interacts with microtubules, and the  in vitro data presented here show that Ug05RP bound to tubulin with a higher affinity compared with Ug11LTS.	bind
26699	2	7151	7	NULL	NULL	0	NULL	Ug05RP	NULL		bind	NULL	high affinity			tubulin	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_46_48197_s_275	15331610	2 Thus, the difference in the speed of apoptosis could be due to the efficiency with which Tat interacts with microtubules, and the  in vitro data presented here show that Ug05RP bound to tubulin with a higher affinity compared with Ug11LTS.	bind
26700	3	7151	7	NULL	NULL	0	NULL	Ug11LTS	NULL		bind	NULL				tubulin	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_46_48197_s_275	15331610	2 Thus, the difference in the speed of apoptosis could be due to the efficiency with which Tat interacts with microtubules, and the  in vitro data presented here show that Ug05RP bound to tubulin with a higher affinity compared with Ug11LTS.	bind
26701	4	7151	7	10	NULL	0	NULL	statement 2	NULL		is higher than	NULL				statement 3	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_46_48197_s_275	15331610	2 Thus, the difference in the speed of apoptosis could be due to the efficiency with which Tat interacts with microtubules, and the  in vitro data presented here show that Ug05RP bound to tubulin with a higher affinity compared with Ug11LTS.	bind
37493	5	7151	7	NULL	NULL	0	NULL	statement 1	NULL	efficiency of	change	NULL				apoptosis	NULL	speed of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_46_48197_s_275	15331610	2 Thus, the difference in the speed of apoptosis could be due to the efficiency with which Tat interacts with microtubules, and the  in vitro data presented here show that Ug05RP bound to tubulin with a higher affinity compared with Ug11LTS.	bind
22405	1	7152	6	13	NULL	NULL	NULL	megalin	GP		bind					Tg	GP	intact			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_43_30377_s_356	10521414	2 Thus, the inhibition produced by the antibody against Tg peptide 1 on megalin binding to intact Tg may be explained by a steric effect.	bind
22406	2	7152	6	13	NULL	NULL	NULL	Tg peptide 1 antibody	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_43_30377_s_356	10521414	2 Thus, the inhibition produced by the antibody against Tg peptide 1 on megalin binding to intact Tg may be explained by a steric effect.	bind
37425	3	7152	6	13	NULL	NULL	NULL	steric effect	Process		cause		may			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_43_30377_s_356	10521414	2 Thus, the inhibition produced by the antibody against Tg peptide 1 on megalin binding to intact Tg may be explained by a steric effect.	bind
26702	1	7152	7	NULL	NULL	0	NULL	 megalin	NULL		bind	NULL				Tg	NULL	intact			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_43_30377_s_356	10521414	2 Thus, the inhibition produced by the antibody against Tg peptide 1 on megalin binding to intact Tg may be explained by a steric effect.	bind
26703	2	7152	7	NULL	NULL	0	NULL	Tg peptide 1 antibody	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_43_30377_s_356	10521414	2 Thus, the inhibition produced by the antibody against Tg peptide 1 on megalin binding to intact Tg may be explained by a steric effect.	bind
26704	3	7152	7	NULL	NULL	0	NULL	steric effect	NULL		cause	NULL	may			statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_43_30377_s_356	10521414	2 Thus, the inhibition produced by the antibody against Tg peptide 1 on megalin binding to intact Tg may be explained by a steric effect.	bind
22407	1	7153	6	13	NULL	NULL	NULL	ConA	GP		bind					insulin receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_12_7833_s_218	9065448	2 Thus, the stimulation of ALPase is not mediated by the binding of ConA to insulin receptors.	bind
22408	2	7153	6	13	NULL	NULL	NULL	ALPase	GP	stimulation of	is not mediated by					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_12_7833_s_218	9065448	2 Thus, the stimulation of ALPase is not mediated by the binding of ConA to insulin receptors.	bind
26705	1	7153	7	NULL	NULL	0	NULL	ConA	NULL		bind	NULL				insulin receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_12_7833_s_218	9065448	2 Thus, the stimulation of ALPase is not mediated by the binding of ConA to insulin receptors.	bind
26706	2	7153	7	NULL	NULL	0	NULL	statement 1	NULL		does not mediate	NULL				ALPase	NULL	stimulation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_12_7833_s_218	9065448	2 Thus, the stimulation of ALPase is not mediated by the binding of ConA to insulin receptors.	bind
22409	1	7154	6	13	NULL	NULL	NULL	CtBP	GP		bind					nNOS	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_51_48262_s_232	11590170	2 Thus, we believe that the binding of CtBP to nNOS plays a role in protein localization rather than regulation of enzymatic activity, suggesting a novel role for nNOS as a targeting molecule.	bind
22410	2	7154	6	13	NULL	NULL	NULL	statement 1	Process		plays a role in					protein localization	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_51_48262_s_232	11590170	2 Thus, we believe that the binding of CtBP to nNOS plays a role in protein localization rather than regulation of enzymatic activity, suggesting a novel role for nNOS as a targeting molecule.	bind
22411	3	7154	6	13	NULL	NULL	NULL	statement 1	Process		does not play a role in					enzymatic activity	Process	regulation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_51_48262_s_232	11590170	2 Thus, we believe that the binding of CtBP to nNOS plays a role in protein localization rather than regulation of enzymatic activity, suggesting a novel role for nNOS as a targeting molecule.	bind
22412	4	7154	6	13	NULL	NULL	NULL	nNOS	GP		acts as a 					targeting molecule	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_51_48262_s_232	11590170	2 Thus, we believe that the binding of CtBP to nNOS plays a role in protein localization rather than regulation of enzymatic activity, suggesting a novel role for nNOS as a targeting molecule.	bind
26707	1	7154	7	NULL	NULL	0	NULL	CtBP	NULL		bind	NULL				nNOS	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_51_48262_s_232	11590170	2 Thus, we believe that the binding of CtBP to nNOS plays a role in protein localization rather than regulation of enzymatic activity, suggesting a novel role for nNOS as a targeting molecule.	bind
26708	2	7154	7	NULL	NULL	0	NULL	statement 1	NULL		plays a role in	NULL				protein localization	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_51_48262_s_232	11590170	2 Thus, we believe that the binding of CtBP to nNOS plays a role in protein localization rather than regulation of enzymatic activity, suggesting a novel role for nNOS as a targeting molecule.	bind
53360	3	7154	7	10	NULL	0	NULL	statement 1	NULL		does not play a role in	NULL				enzymatic activity	NULL	regulation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_51_48262_s_232	11590170	2 Thus, we believe that the binding of CtBP to nNOS plays a role in protein localization rather than regulation of enzymatic activity, suggesting a novel role for nNOS as a targeting molecule.	bind
53361	4	7154	7	10	NULL	0	NULL	nNOS	NULL		acts as	NULL				targeting molecule	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_51_48262_s_232	11590170	2 Thus, we believe that the binding of CtBP to nNOS plays a role in protein localization rather than regulation of enzymatic activity, suggesting a novel role for nNOS as a targeting molecule.	bind
22413	1	7155	6	13	NULL	NULL	NULL	TM	GP		bind					thrombin	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_1_41_s_20	12522119	2 TM binds thrombin and alters its active site specificity to facilitate proteolytic activation of protein C, a potent inhibitor of the coagulation cascade.	bind
22414	3	7155	6	13	NULL	NULL	NULL	statement 2	Process		facilitates					protein C	GP	proteolytic activation of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_1_41_s_20	12522119	2 TM binds thrombin and alters its active site specificity to facilitate proteolytic activation of protein C, a potent inhibitor of the coagulation cascade.	bind
22415	4	7155	6	13	NULL	NULL	NULL	Protein C	GP		is an inhibitor of		potent			coagulation cascade	Process	inhibitor of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_1_41_s_20	12522119	2 TM binds thrombin and alters its active site specificity to facilitate proteolytic activation of protein C, a potent inhibitor of the coagulation cascade.	bind
22416	2	7155	6	13	NULL	NULL	NULL	statement 1	Process		alters					thrombin	GP	specificity of 	active site		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_1_41_s_20	12522119	2 TM binds thrombin and alters its active site specificity to facilitate proteolytic activation of protein C, a potent inhibitor of the coagulation cascade.	bind
26713	1	7155	7	NULL	NULL	0	NULL	TM	NULL		binds	NULL				thrombin	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_92_1_41_s_20	12522119	2 TM binds thrombin and alters its active site specificity to facilitate proteolytic activation of protein C, a potent inhibitor of the coagulation cascade.	bind
26716	2	7155	7	NULL	NULL	0	NULL	statement 1	NULL		alter	NULL				thrombin	NULL	specificity of	active site		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_1_41_s_20	12522119	2 TM binds thrombin and alters its active site specificity to facilitate proteolytic activation of protein C, a potent inhibitor of the coagulation cascade.	bind
26718	3	7155	7	NULL	NULL	0	NULL	statement 2	NULL		facilitate	NULL				protein C	NULL	proteolytic activation of			NULL		0	NULL	NULL	NULL	gw70_circulationres_92_1_41_s_20	12522119	2 TM binds thrombin and alters its active site specificity to facilitate proteolytic activation of protein C, a potent inhibitor of the coagulation cascade.	bind
26721	4	7155	7	10	NULL	0	NULL	protein C	NULL		is an inhibitor of	NULL	potent			coagulation cascade	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_1_41_s_20	12522119	2 TM binds thrombin and alters its active site specificity to facilitate proteolytic activation of protein C, a potent inhibitor of the coagulation cascade.	bind
22417	1	7156	6	13	NULL	NULL	NULL	rHSF-1	GP		bind					IL1B	GP			promoter fragments	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_40_24874_s_34	8926278	2 To analyze the binding of rHSF-1 to  IL1B promoter fragments, probes were labeled by end filling with Klenow fragment using [32]dCTP at 6,000 Ci/mmol (DuPont NEN) to an activity of 100,000 cpm/ng and incubated (0.2 ng each) with rHSF-1 (0.7 mug), poly(DI.	bind
26722	1	7156	7	10	NULL	0	NULL	rHSF-1	NULL		bind	NULL				IL1B	NULL			promoter fragments	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_40_24874_s_34	8926278	2 To analyze the binding of rHSF-1 to  IL1B promoter fragments, probes were labeled by end filling with Klenow fragment using [32]dCTP at 6,000 Ci/mmol (DuPont NEN) to an activity of 100,000 cpm/ng and incubated (0.2 ng each) with rHSF-1 (0.7 mug), poly(DI.	bind
22418	1	7157	6	13	NULL	NULL	NULL	CB1	GP		bind					His6-sCD4	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_508_1_67_s_168	11707270	2 to displace the binding of PDPs CB1 and CB8 to His6-sCD4 was studied by using an ELISA inhibition assay.	bind
22419	2	7157	6	13	NULL	NULL	NULL	CB8	GP		bind					His6-sCD4	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_508_1_67_s_168	11707270	2 to displace the binding of PDPs CB1 and CB8 to His6-sCD4 was studied by using an ELISA inhibition assay.	bind
37426	3	7157	6	13	NULL	NULL	NULL	CB1	GP		is a type of					PDP	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_508_1_67_s_168	11707270	2 to displace the binding of PDPs CB1 and CB8 to His6-sCD4 was studied by using an ELISA inhibition assay.	bind
37427	4	7157	6	13	NULL	NULL	NULL	CB8	GP		is a type of					PDP	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_508_1_67_s_168	11707270	2 to displace the binding of PDPs CB1 and CB8 to His6-sCD4 was studied by using an ELISA inhibition assay.	bind
26723	1	7157	7	NULL	NULL	0	NULL	 CB1	NULL		bind	NULL				His6-sCD4	NULL				NULL		NULL	NULL	NULL	NULL	gw60_febslett_508_1_67_s_168	11707270	2 to displace the binding of PDPs CB1 and CB8 to His6-sCD4 was studied by using an ELISA inhibition assay.	bind
26725	2	7157	7	NULL	NULL	0	NULL	 CB8	NULL		bind	NULL				His6-sCD4 	NULL				NULL		NULL	NULL	NULL	NULL	gw60_febslett_508_1_67_s_168	11707270	2 to displace the binding of PDPs CB1 and CB8 to His6-sCD4 was studied by using an ELISA inhibition assay.	bind
37494	3	7157	7	NULL	NULL	0	NULL	CB1	NULL		is a type of	NULL				PDPs	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_508_1_67_s_168	11707270	2 to displace the binding of PDPs CB1 and CB8 to His6-sCD4 was studied by using an ELISA inhibition assay.	bind
37495	4	7157	7	NULL	NULL	0	NULL	CB8	NULL		is a type of	NULL				PDPs	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_508_1_67_s_168	11707270	2 to displace the binding of PDPs CB1 and CB8 to His6-sCD4 was studied by using an ELISA inhibition assay.	bind
22420	1	7159	6	13	NULL	NULL	NULL	integrin	GP		mediates					Raf-1	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_42_27268_s_69	9765250	2 To more directly address the question of whether interaction with Ras is required for integrin-mediated activation of Raf-1, cells were transiently transfected with plasmids encoding either wild-type Raf (Raf-WT) or a mutant allele containing an arginine to leucine substitution at position 89, within the Ras binding domain (Raf-R89L) ( 25).	bind
26729	1	7159	7	NULL	NULL	0	NULL	 integrin	NULL		mediates	NULL				Raf-1	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_42_27268_s_69	9765250	2 To more directly address the question of whether interaction with Ras is required for integrin-mediated activation of Raf-1, cells were transiently transfected with plasmids encoding either wild-type Raf (Raf-WT) or a mutant allele containing an arginine to leucine substitution at position 89, within the Ras binding domain (Raf-R89L) ( 25).	bind
22421	1	7160	6	13	NULL	NULL	NULL	TRP	GP		does not bind					DNA	NucleicAcid			TATA	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_1_122_s_239	10617594	2 TRP does not bind to TATA-DNA but does interact with general transcription factors TFIIA and TFIIB.	bind
22422	2	7160	6	13	NULL	NULL	NULL	TRP	GP		interacts with					TFIIA 	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_1_122_s_239	10617594	2 TRP does not bind to TATA-DNA but does interact with general transcription factors TFIIA and TFIIB.	bind
22423	3	7160	6	13	NULL	NULL	NULL	TRP	GP		interacts with					TFIIB	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_1_122_s_239	10617594	2 TRP does not bind to TATA-DNA but does interact with general transcription factors TFIIA and TFIIB.	bind
37428	4	7160	6	13	NULL	NULL	NULL	TFIIA	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_1_122_s_239	10617594	2 TRP does not bind to TATA-DNA but does interact with general transcription factors TFIIA and TFIIB.	bind
37429	5	7160	6	13	NULL	NULL	NULL	TFIIB	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_1_122_s_239	10617594	2 TRP does not bind to TATA-DNA but does interact with general transcription factors TFIIA and TFIIB.	bind
26731	1	7160	7	NULL	NULL	0	NULL	TRP	NULL		does not bind	NULL				 DNA	NULL			TATA	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_1_122_s_239	10617594	2 TRP does not bind to TATA-DNA but does interact with general transcription factors TFIIA and TFIIB.	bind
26732	2	7160	7	NULL	NULL	0	NULL	TRP	NULL		interacts with	NULL				TFIIA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_1_122_s_239	10617594	2 TRP does not bind to TATA-DNA but does interact with general transcription factors TFIIA and TFIIB.	bind
26733	3	7160	7	NULL	NULL	0	NULL	TRP	NULL		interacts with	NULL				TFIIB	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_1_122_s_239	10617594	2 TRP does not bind to TATA-DNA but does interact with general transcription factors TFIIA and TFIIB.	bind
26734	4	7160	7	NULL	NULL	0	NULL	TFIIA	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_1_122_s_239	10617594	2 TRP does not bind to TATA-DNA but does interact with general transcription factors TFIIA and TFIIB.	bind
26735	5	7160	7	NULL	NULL	0	NULL	TFIIB	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_1_122_s_239	10617594	2 TRP does not bind to TATA-DNA but does interact with general transcription factors TFIIA and TFIIB.	bind
22424	1	7161	6	13	NULL	NULL	NULL	GDP	Chemical		bind					Ras	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_8_4392_s_26	9468490	2 Two GAPs, NF1 and RasGAP, form stable complexes with the GDP-bound form of Ras in the presence of aluminum fluoride, indicating that it also mimics the transition state of GTP hydrolysis in low molecular weight GTP-binding proteins.	bind
22425	2	7161	6	13	NULL	NULL	NULL	NF1	GP		form stable complex with					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_8_4392_s_26	9468490	2 Two GAPs, NF1 and RasGAP, form stable complexes with the GDP-bound form of Ras in the presence of aluminum fluoride, indicating that it also mimics the transition state of GTP hydrolysis in low molecular weight GTP-binding proteins.	bind
22426	3	7161	6	13	NULL	NULL	NULL	RasGAP	GP		form stable complex with					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_8_4392_s_26	9468490	2 Two GAPs, NF1 and RasGAP, form stable complexes with the GDP-bound form of Ras in the presence of aluminum fluoride, indicating that it also mimics the transition state of GTP hydrolysis in low molecular weight GTP-binding proteins.	bind
22427	4	7161	6	13	NULL	NULL	NULL	statement 2	Process		occurs in presence of					aluminium fluoride	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_8_4392_s_26	9468490	2 Two GAPs, NF1 and RasGAP, form stable complexes with the GDP-bound form of Ras in the presence of aluminum fluoride, indicating that it also mimics the transition state of GTP hydrolysis in low molecular weight GTP-binding proteins.	bind
22428	5	7161	6	13	NULL	NULL	NULL	statement 3	Process		occurs in presence of					aluminium fluoride	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_8_4392_s_26	9468490	2 Two GAPs, NF1 and RasGAP, form stable complexes with the GDP-bound form of Ras in the presence of aluminum fluoride, indicating that it also mimics the transition state of GTP hydrolysis in low molecular weight GTP-binding proteins.	bind
26920	1	7161	7	10	NULL	0	NULL	NF1	NULL		forms stable complex with	NULL				statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_8_4392_s_26	9468490	2 Two GAPs, NF1 and RasGAP, form stable complexes with the GDP-bound form of Ras in the presence of aluminum fluoride, indicating that it also mimics the transition state of GTP hydrolysis in low molecular weight GTP-binding proteins.	bind
26921	2	7161	7	NULL	NULL	0	NULL	RasGAP	NULL		forms stable complex with	NULL				GDP-bound Ras	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_8_4392_s_26	9468490	2 Two GAPs, NF1 and RasGAP, form stable complexes with the GDP-bound form of Ras in the presence of aluminum fluoride, indicating that it also mimics the transition state of GTP hydrolysis in low molecular weight GTP-binding proteins.	bind
26922	3	7161	7	NULL	NULL	0	NULL	statement 1	NULL		in presence of	NULL				aluminum fluoride	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_8_4392_s_26	9468490	2 Two GAPs, NF1 and RasGAP, form stable complexes with the GDP-bound form of Ras in the presence of aluminum fluoride, indicating that it also mimics the transition state of GTP hydrolysis in low molecular weight GTP-binding proteins.	bind
26923	4	7161	7	NULL	NULL	0	NULL	statement 2	NULL		in presence of	NULL				aluminum fluoride	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_8_4392_s_26	9468490	2 Two GAPs, NF1 and RasGAP, form stable complexes with the GDP-bound form of Ras in the presence of aluminum fluoride, indicating that it also mimics the transition state of GTP hydrolysis in low molecular weight GTP-binding proteins.	bind
46449	5	7161	7	10	NULL	0	NULL	GDP	NULL		bind	NULL				Ras	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_8_4392_s_26	9468490	2 Two GAPs, NF1 and RasGAP, form stable complexes with the GDP-bound form of Ras in the presence of aluminum fluoride, indicating that it also mimics the transition state of GTP hydrolysis in low molecular weight GTP-binding proteins.	bind
22531	1	7162	6	13	NULL	NULL	NULL	CBD23 construct	GP	mutant	does not bind			W316A/W374A		gelatin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_41_43336_s_222	15292230	2 Using a CBD23 construct with the tryptophan mutations W316A/W374A that no longerR binds gelatin nor blocks MMP-2 gelatinolytic and collagenolytic activities in competition experiments, we specifically confirmed the importance of the collagen binding properties of the CBD in collagen and gelatin cleavage by MMP-2.	bind
22532	2	7162	6	13	NULL	NULL	NULL	MMP-2	GP		cleaves					collagen	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_41_43336_s_222	15292230	2 Using a CBD23 construct with the tryptophan mutations W316A/W374A that no longerR binds gelatin nor blocks MMP-2 gelatinolytic and collagenolytic activities in competition experiments, we specifically confirmed the importance of the collagen binding properties of the CBD in collagen and gelatin cleavage by MMP-2.	bind
22533	3	7162	6	13	NULL	NULL	NULL	MMP-2	GP		cleaves					gelatin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_41_43336_s_222	15292230	2 Using a CBD23 construct with the tryptophan mutations W316A/W374A that no longerR binds gelatin nor blocks MMP-2 gelatinolytic and collagenolytic activities in competition experiments, we specifically confirmed the importance of the collagen binding properties of the CBD in collagen and gelatin cleavage by MMP-2.	bind
22534	4	7162	6	13	NULL	NULL	NULL	CBD23 construct	GP	mutant	does not block			W316A/W374A		MMP-2	GP	gelatinolytic activity of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_41_43336_s_222	15292230	2 Using a CBD23 construct with the tryptophan mutations W316A/W374A that no longerR binds gelatin nor blocks MMP-2 gelatinolytic and collagenolytic activities in competition experiments, we specifically confirmed the importance of the collagen binding properties of the CBD in collagen and gelatin cleavage by MMP-2.	bind
22535	5	7162	6	13	NULL	NULL	NULL	CBD23 construct	GP	mutant	does not block			W316A/W374A		MMP-2	GP	collagenolytic activity of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_41_43336_s_222	15292230	2 Using a CBD23 construct with the tryptophan mutations W316A/W374A that no longerR binds gelatin nor blocks MMP-2 gelatinolytic and collagenolytic activities in competition experiments, we specifically confirmed the importance of the collagen binding properties of the CBD in collagen and gelatin cleavage by MMP-2.	bind
22536	6	7162	6	13	NULL	NULL	NULL				bind			CBD		collagen	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_41_43336_s_222	15292230	2 Using a CBD23 construct with the tryptophan mutations W316A/W374A that no longerR binds gelatin nor blocks MMP-2 gelatinolytic and collagenolytic activities in competition experiments, we specifically confirmed the importance of the collagen binding properties of the CBD in collagen and gelatin cleavage by MMP-2.	bind
22537	7	7162	6	13	NULL	NULL	NULL	statement 6	Process		plays a role in					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_41_43336_s_222	15292230	2 Using a CBD23 construct with the tryptophan mutations W316A/W374A that no longerR binds gelatin nor blocks MMP-2 gelatinolytic and collagenolytic activities in competition experiments, we specifically confirmed the importance of the collagen binding properties of the CBD in collagen and gelatin cleavage by MMP-2.	bind
22538	8	7162	6	13	NULL	NULL	NULL	statement 6	Process		plays a role in					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_41_43336_s_222	15292230	2 Using a CBD23 construct with the tryptophan mutations W316A/W374A that no longerR binds gelatin nor blocks MMP-2 gelatinolytic and collagenolytic activities in competition experiments, we specifically confirmed the importance of the collagen binding properties of the CBD in collagen and gelatin cleavage by MMP-2.	bind
26926	1	7162	7	NULL	NULL	0	NULL	CBD	NULL		binds	NULL				collagen	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_41_43336_s_222	15292230	2 Using a CBD23 construct with the tryptophan mutations W316A/W374A that no longerR binds gelatin nor blocks MMP-2 gelatinolytic and collagenolytic activities in competition experiments, we specifically confirmed the importance of the collagen binding properties of the CBD in collagen and gelatin cleavage by MMP-2.	bind
26927	2	7162	7	NULL	NULL	0	NULL	MMP-2	NULL		cleaves	NULL				gelatin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_41_43336_s_222	15292230	2 Using a CBD23 construct with the tryptophan mutations W316A/W374A that no longerR binds gelatin nor blocks MMP-2 gelatinolytic and collagenolytic activities in competition experiments, we specifically confirmed the importance of the collagen binding properties of the CBD in collagen and gelatin cleavage by MMP-2.	bind
27857	3	7162	7	NULL	NULL	0	NULL	 CBD23 construct	NULL	mutant	does not bind	NULL		W316A/W374A		gelatin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_41_43336_s_222	15292230	2 Using a CBD23 construct with the tryptophan mutations W316A/W374A that no longerR binds gelatin nor blocks MMP-2 gelatinolytic and collagenolytic activities in competition experiments, we specifically confirmed the importance of the collagen binding properties of the CBD in collagen and gelatin cleavage by MMP-2.	bind
27858	5	7162	7	10	NULL	0	NULL	CBD23 construct	NULL	mutant	does not block	NULL		W316A/W374A		MMP-2	NULL	gelatinolytic activity of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_41_43336_s_222	15292230	2 Using a CBD23 construct with the tryptophan mutations W316A/W374A that no longerR binds gelatin nor blocks MMP-2 gelatinolytic and collagenolytic activities in competition experiments, we specifically confirmed the importance of the collagen binding properties of the CBD in collagen and gelatin cleavage by MMP-2.	bind
27859	7	7162	7	10	NULL	0	NULL	CBD23 construct	NULL	mutant	does not block	NULL		W316A/W374A		MMP-2	NULL	collagenolytic activity of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_41_43336_s_222	15292230	2 Using a CBD23 construct with the tryptophan mutations W316A/W374A that no longerR binds gelatin nor blocks MMP-2 gelatinolytic and collagenolytic activities in competition experiments, we specifically confirmed the importance of the collagen binding properties of the CBD in collagen and gelatin cleavage by MMP-2.	bind
37587	4	7162	7	10	NULL	0	NULL	MMP-2	NULL		cleaves	NULL				collagen	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_41_43336_s_222	15292230	2 Using a CBD23 construct with the tryptophan mutations W316A/W374A that no longerR binds gelatin nor blocks MMP-2 gelatinolytic and collagenolytic activities in competition experiments, we specifically confirmed the importance of the collagen binding properties of the CBD in collagen and gelatin cleavage by MMP-2.	bind
37588	6	7162	7	10	NULL	0	NULL	statement 1	NULL		plays a role in	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_41_43336_s_222	15292230	2 Using a CBD23 construct with the tryptophan mutations W316A/W374A that no longerR binds gelatin nor blocks MMP-2 gelatinolytic and collagenolytic activities in competition experiments, we specifically confirmed the importance of the collagen binding properties of the CBD in collagen and gelatin cleavage by MMP-2.	bind
53362	8	7162	7	10	NULL	0	NULL	statement 1	NULL		plays a role in	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_41_43336_s_222	15292230	2 Using a CBD23 construct with the tryptophan mutations W316A/W374A that no longerR binds gelatin nor blocks MMP-2 gelatinolytic and collagenolytic activities in competition experiments, we specifically confirmed the importance of the collagen binding properties of the CBD in collagen and gelatin cleavage by MMP-2.	bind
22429	1	7163	6	13	NULL	NULL	NULL	GTP	Chemical		bind					Rho	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_38_23022_s_26	8798490	2 Using the two hybrid system, we also isolated another molecule showing binding to GTP-bound forms of Rho and Rac.	bind
22430	2	7163	6	13	NULL	NULL	NULL	GTP	Chemical		bind					Rac	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_38_23022_s_26	8798490	2 Using the two hybrid system, we also isolated another molecule showing binding to GTP-bound forms of Rho and Rac.	bind
26928	1	7163	7	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				Rho	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_38_23022_s_26	8798490	2 Using the two hybrid system, we also isolated another molecule showing binding to GTP-bound forms of Rho and Rac.	bind
26929	2	7163	7	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				Rac	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_38_23022_s_26	8798490	2 Using the two hybrid system, we also isolated another molecule showing binding to GTP-bound forms of Rho and Rac.	bind
22431	1	7165	6	13	NULL	NULL	NULL	ETO-1 protein	GP	arabidopsis	bind			BTB domain		CUL3a	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_19_18810_s_61	15749712	2 Wang  et al. ( ) provided further support with the discovery that the  Arabidopsis ethylene  overproducer (ETO)-1 protein contains a BTB domain that binds CUL3a.	bind
22432	2	7165	6	13	NULL	NULL	NULL	ETO-1	GP		is					ethylene overproducer 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_19_18810_s_61	15749712	2 Wang  et al. ( ) provided further support with the discovery that the  Arabidopsis ethylene  overproducer (ETO)-1 protein contains a BTB domain that binds CUL3a.	bind
26930	1	7165	7	NULL	NULL	0	NULL	ETO-1 protein 	NULL	Arabidopsis	binds	NULL		BTB domain		CUL3a	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_19_18810_s_61	15749712	2 Wang  et al. ( ) provided further support with the discovery that the  Arabidopsis ethylene  overproducer (ETO)-1 protein contains a BTB domain that binds CUL3a.	bind
26931	2	7165	7	NULL	NULL	0	NULL	ETO-1 protein	NULL		is	NULL				ethylene overproducer-1 protein	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_19_18810_s_61	15749712	2 Wang  et al. ( ) provided further support with the discovery that the  Arabidopsis ethylene  overproducer (ETO)-1 protein contains a BTB domain that binds CUL3a.	bind
22433	1	7166	6	13	NULL	NULL	NULL	Cox17	GP		exist within a					binuclear thiolate center	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_48_37582_s_237	10970896	2 We had proposed that the two Cu(I) ions bound to Cox17 purified as a GST fusion exist within a binuclear thiolate center with either four or five thiolate ligands ( 14).	bind
22434	2	7166	6	13	NULL	NULL	NULL	Cu(I) ions	Chemical		bind					Cox17	GP	purified			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_48_37582_s_237	10970896	2 We had proposed that the two Cu(I) ions bound to Cox17 purified as a GST fusion exist within a binuclear thiolate center with either four or five thiolate ligands ( 14).	bind
37430	3	7166	6	13	NULL	NULL	NULL	Cox17	GP		contains					thiolate ligands	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_48_37582_s_237	10970896	2 We had proposed that the two Cu(I) ions bound to Cox17 purified as a GST fusion exist within a binuclear thiolate center with either four or five thiolate ligands ( 14).	bind
46450	4	7166	6	13	NULL	NULL	NULL	Cox17	GP		is a type of					GST fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_48_37582_s_237	10970896	2 We had proposed that the two Cu(I) ions bound to Cox17 purified as a GST fusion exist within a binuclear thiolate center with either four or five thiolate ligands ( 14).	bind
26932	1	7166	7	10	NULL	0	NULL	Cu(I) ions	NULL		bind	NULL				Cox17	NULL	purified 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_48_37582_s_237	10970896	2 We had proposed that the two Cu(I) ions bound to Cox17 purified as a GST fusion exist within a binuclear thiolate center with either four or five thiolate ligands ( 14).	bind
26933	2	7166	7	NULL	NULL	0	NULL	 Cox17	NULL		exist within	NULL				binuclear thiolate center	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_48_37582_s_237	10970896	2 We had proposed that the two Cu(I) ions bound to Cox17 purified as a GST fusion exist within a binuclear thiolate center with either four or five thiolate ligands ( 14).	bind
26934	3	7166	7	NULL	NULL	0	NULL	Cox17	NULL		contains	NULL				thiolate ligands	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_48_37582_s_237	10970896	2 We had proposed that the two Cu(I) ions bound to Cox17 purified as a GST fusion exist within a binuclear thiolate center with either four or five thiolate ligands ( 14).	bind
46451	4	7166	7	10	NULL	0	NULL	Cox17	NULL		is a type of	NULL				GST fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_48_37582_s_237	10970896	2 We had proposed that the two Cu(I) ions bound to Cox17 purified as a GST fusion exist within a binuclear thiolate center with either four or five thiolate ligands ( 14).	bind
22435	1	7167	6	13	NULL	NULL	NULL	hnRNP C	GP		bind									29-base instability element 	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_2_1119_s_295	11042220	2 We have proposed that the stable phase was a consequence of hnRNP C binding to the 29-base instability element that prevented RNase attack.	bind
22436	2	7167	6	13	NULL	NULL	NULL	statement 1	Process		prevents					RNase attack	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_2_1119_s_295	11042220	2 We have proposed that the stable phase was a consequence of hnRNP C binding to the 29-base instability element that prevented RNase attack.	bind
26935	1	7167	7	NULL	NULL	0	NULL	hnRNP C	NULL		bind	NULL					NULL			29-base instability element	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_2_1119_s_295	11042220	2 We have proposed that the stable phase was a consequence of hnRNP C binding to the 29-base instability element that prevented RNase attack.	bind
26936	2	7167	7	NULL	NULL	0	NULL	statement 1	NULL		prevents	NULL				RNase attack	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_2_1119_s_295	11042220	2 We have proposed that the stable phase was a consequence of hnRNP C binding to the 29-base instability element that prevented RNase attack.	bind
22437	1	7168	6	13	NULL	NULL	NULL	LDL	GP		bind					LRP	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_15_13350_s_180	12566436	2 We show here that binding of LDL to LRP is also required for 12/15 -lipoxygenasetranslocation (Fig.  3).	bind
22438	2	7168	6	13	NULL	NULL	NULL	statement 1	Process		is required for					12/15 -lipoxygenase	GP	translocation of 			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_15_13350_s_180	12566436	2 We show here that binding of LDL to LRP is also required for 12/15 -lipoxygenasetranslocation (Fig.  3).	bind
26937	1	7168	7	NULL	NULL	0	NULL	LDL	NULL		bind	NULL				LRP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_15_13350_s_180	12566436	2 We show here that binding of LDL to LRP is also required for 12/15 -lipoxygenasetranslocation (Fig.  3).	bind
26938	2	7168	7	NULL	NULL	0	NULL	statement 1	NULL		is required for	NULL				12/15 -lipoxygenase	NULL	translocation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_15_13350_s_180	12566436	2 We show here that binding of LDL to LRP is also required for 12/15 -lipoxygenasetranslocation (Fig.  3).	bind
37434	2	7169	6	13	NULL	NULL	NULL	Galphaq	GP		interacts with			Q209L		statement 1	GP				NULL	cultured cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_6050_s_217	12427730	2 We thus used this assay to examine interactions between Galphaq-Q209L and a Galphaq binding-defective mutant of GRK2 in cultured cells (Fig.  4).	bind
46452	1	7169	6	13	NULL	NULL	NULL	GRK2	GP	defective mutant	bind					Galphaq	GP				NULL	cultured cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_6050_s_217	12427730	2 We thus used this assay to examine interactions between Galphaq-Q209L and a Galphaq binding-defective mutant of GRK2 in cultured cells (Fig.  4).	bind
26939	2	7169	7	10	NULL	0	NULL	Galphaq	NULL		interacts with	NULL		Q209L		statement 1	NULL				NULL	cultured cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_6050_s_217	12427730	2 We thus used this assay to examine interactions between Galphaq-Q209L and a Galphaq binding-defective mutant of GRK2 in cultured cells (Fig.  4).	bind
46453	1	7169	7	10	NULL	0	NULL	GRK2	NULL	defective mutant	bind	NULL				Galphaq	NULL				NULL	cultured cells	0	NULL	NULL	NULL	gw70_jbiolchem_278_8_6050_s_217	12427730	2 We thus used this assay to examine interactions between Galphaq-Q209L and a Galphaq binding-defective mutant of GRK2 in cultured cells (Fig.  4).	bind
22439	1	7170	6	13	NULL	NULL	NULL	Diva	GP		interacts with					Apaf-1	GP				NULL	mammalian cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_49_32479_s_185	9829980	2 We verified the interaction between Diva and Apaf-1 in mammalian cells and tested whether Diva might block the binding of Bcl-XL to Apaf-1, because Bcl-XL can also interact with Apaf-1 ( 10,  11).	bind
22440	2	7170	6	13	NULL	NULL	NULL	Bcl-XL	GP		interacts with					Apaf1	GP				NULL	mammalian cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_49_32479_s_185	9829980	2 We verified the interaction between Diva and Apaf-1 in mammalian cells and tested whether Diva might block the binding of Bcl-XL to Apaf-1, because Bcl-XL can also interact with Apaf-1 ( 10,  11).	bind
46454	3	7170	6	13	NULL	NULL	NULL	Diva	GP		block		may			statement 2	Process				NULL	mammalian cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_49_32479_s_185	9829980	2 We verified the interaction between Diva and Apaf-1 in mammalian cells and tested whether Diva might block the binding of Bcl-XL to Apaf-1, because Bcl-XL can also interact with Apaf-1 ( 10,  11).	bind
26940	1	7170	7	NULL	NULL	0	NULL	 Diva	NULL		interacts with	NULL				Apaf-1	NULL				NULL	mammalian cells	0	NULL	NULL	NULL	gw60_jbiolchem_273_49_32479_s_185	9829980	2 We verified the interaction between Diva and Apaf-1 in mammalian cells and tested whether Diva might block the binding of Bcl-XL to Apaf-1, because Bcl-XL can also interact with Apaf-1 ( 10,  11).	bind
26941	2	7170	7	NULL	NULL	0	NULL	 Bcl-XL	NULL		interacts with	NULL				Apaf-1 	NULL				NULL	mammalian cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_49_32479_s_185	9829980	2 We verified the interaction between Diva and Apaf-1 in mammalian cells and tested whether Diva might block the binding of Bcl-XL to Apaf-1, because Bcl-XL can also interact with Apaf-1 ( 10,  11).	bind
26942	3	7170	7	NULL	NULL	0	NULL	Diva	NULL		block	NULL	may			statement 2	NULL				NULL	mammalian cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_49_32479_s_185	9829980	2 We verified the interaction between Diva and Apaf-1 in mammalian cells and tested whether Diva might block the binding of Bcl-XL to Apaf-1, because Bcl-XL can also interact with Apaf-1 ( 10,  11).	bind
22441	1	7171	6	13	NULL	NULL	NULL	Grb7	GP		bind		specifically	SH2 domain		erbB2	GP				NULL	lysates of control cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_13_7717_s_153	9516479	2 Western blot analysis using specific antibodies revealed that the Grb7 SH2 domain specifically bound erbB2 and erbB3 from lysates of control cells, presumably because of the basal phosphorylation of these erbB receptors observed in ZR-75-1 cells ( 45), but this interaction was increased significantly when lysates from heregulin-stimulated cells were used (Fig.  3 A).	bind
22442	2	7171	6	13	NULL	NULL	NULL	Grb7	GP		bind		specifically	SH2 domain		erbB3	GP				NULL	lysates of control cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_13_7717_s_153	9516479	2 Western blot analysis using specific antibodies revealed that the Grb7 SH2 domain specifically bound erbB2 and erbB3 from lysates of control cells, presumably because of the basal phosphorylation of these erbB receptors observed in ZR-75-1 cells ( 45), but this interaction was increased significantly when lysates from heregulin-stimulated cells were used (Fig.  3 A).	bind
22539	3	7171	6	13	NULL	NULL	NULL	erbB receptors	GP	basal phosphorylation of 	cause		presumably			statement 1	Process				NULL	ZR-75-1 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_13_7717_s_153	9516479	2 Western blot analysis using specific antibodies revealed that the Grb7 SH2 domain specifically bound erbB2 and erbB3 from lysates of control cells, presumably because of the basal phosphorylation of these erbB receptors observed in ZR-75-1 cells ( 45), but this interaction was increased significantly when lysates from heregulin-stimulated cells were used (Fig.  3 A).	bind
22540	4	7171	6	13	NULL	NULL	NULL	erbB receptors	GP	basal phosphorylation of 	cause		presumably			statement 2	Process				NULL	ZR-75-1 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_13_7717_s_153	9516479	2 Western blot analysis using specific antibodies revealed that the Grb7 SH2 domain specifically bound erbB2 and erbB3 from lysates of control cells, presumably because of the basal phosphorylation of these erbB receptors observed in ZR-75-1 cells ( 45), but this interaction was increased significantly when lysates from heregulin-stimulated cells were used (Fig.  3 A).	bind
22541	5	7171	6	13	NULL	NULL	NULL	Grb7	GP		bind		specifically	SH2 domain		erbB2 receptors	GP				NULL	lysates from heregulin-stimulated cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_13_7717_s_153	9516479	2 Western blot analysis using specific antibodies revealed that the Grb7 SH2 domain specifically bound erbB2 and erbB3 from lysates of control cells, presumably because of the basal phosphorylation of these erbB receptors observed in ZR-75-1 cells ( 45), but this interaction was increased significantly when lysates from heregulin-stimulated cells were used (Fig.  3 A).	bind
22542	6	7171	6	13	NULL	NULL	NULL	Grb7	GP		bind		specifically	SH2 domain		erbB3 receptor	GP				NULL	lysates from heregulin-stimulated cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_13_7717_s_153	9516479	2 Western blot analysis using specific antibodies revealed that the Grb7 SH2 domain specifically bound erbB2 and erbB3 from lysates of control cells, presumably because of the basal phosphorylation of these erbB receptors observed in ZR-75-1 cells ( 45), but this interaction was increased significantly when lysates from heregulin-stimulated cells were used (Fig.  3 A).	bind
22543	7	7171	6	13	NULL	NULL	NULL	statement 5	Process		is increased as compared to		significantly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_13_7717_s_153	9516479	2 Western blot analysis using specific antibodies revealed that the Grb7 SH2 domain specifically bound erbB2 and erbB3 from lysates of control cells, presumably because of the basal phosphorylation of these erbB receptors observed in ZR-75-1 cells ( 45), but this interaction was increased significantly when lysates from heregulin-stimulated cells were used (Fig.  3 A).	bind
46808	8	7171	6	13	NULL	NULL	NULL	statement 6	Process		is increased as compared to		significantly			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_13_7717_s_153	9516479	2 Western blot analysis using specific antibodies revealed that the Grb7 SH2 domain specifically bound erbB2 and erbB3 from lysates of control cells, presumably because of the basal phosphorylation of these erbB receptors observed in ZR-75-1 cells ( 45), but this interaction was increased significantly when lysates from heregulin-stimulated cells were used (Fig.  3 A).	bind
26943	1	7171	7	10	NULL	0	NULL	Grb7 	NULL		bind	NULL	specifically	SH2 domain		erbB2 	NULL				NULL	lysates of control cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_13_7717_s_153	9516479	2 Western blot analysis using specific antibodies revealed that the Grb7 SH2 domain specifically bound erbB2 and erbB3 from lysates of control cells, presumably because of the basal phosphorylation of these erbB receptors observed in ZR-75-1 cells ( 45), but this interaction was increased significantly when lysates from heregulin-stimulated cells were used (Fig.  3 A).	bind
26944	2	7171	7	10	NULL	0	NULL	Grb7	NULL		bind	NULL	specifically	SH2 domain		erbB3	NULL				NULL	lysates of control cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_13_7717_s_153	9516479	2 Western blot analysis using specific antibodies revealed that the Grb7 SH2 domain specifically bound erbB2 and erbB3 from lysates of control cells, presumably because of the basal phosphorylation of these erbB receptors observed in ZR-75-1 cells ( 45), but this interaction was increased significantly when lysates from heregulin-stimulated cells were used (Fig.  3 A).	bind
26945	3	7171	7	10	NULL	0	NULL	statement 1			because of		presumably			erbB receptors 		basal phosphorylation of			NULL	ZR-75-1 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_13_7717_s_153	9516479	2 Western blot analysis using specific antibodies revealed that the Grb7 SH2 domain specifically bound erbB2 and erbB3 from lysates of control cells, presumably because of the basal phosphorylation of these erbB receptors observed in ZR-75-1 cells ( 45), but this interaction was increased significantly when lysates from heregulin-stimulated cells were used (Fig.  3 A).	bind
26947	4	7171	7	10	NULL	0	NULL	statement 2			because of		presumably			erbB receptors		basal phosphorylation of			NULL	ZR-75-1 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_13_7717_s_153	9516479	2 Western blot analysis using specific antibodies revealed that the Grb7 SH2 domain specifically bound erbB2 and erbB3 from lysates of control cells, presumably because of the basal phosphorylation of these erbB receptors observed in ZR-75-1 cells ( 45), but this interaction was increased significantly when lysates from heregulin-stimulated cells were used (Fig.  3 A).	bind
26948	6	7171	7	NULL	NULL	0	NULL	Grb7			bind			SH2 domain		erbB3					NULL	heregulin-stimulated cells 	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_13_7717_s_153	9516479	2 Western blot analysis using specific antibodies revealed that the Grb7 SH2 domain specifically bound erbB2 and erbB3 from lysates of control cells, presumably because of the basal phosphorylation of these erbB receptors observed in ZR-75-1 cells ( 45), but this interaction was increased significantly when lysates from heregulin-stimulated cells were used (Fig.  3 A).	bind
54109	5	7171	7	NULL	NULL	0	NULL	Grb7			bind			SH2 domain		erbB2					NULL	 heregulin-stimulated cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_13_7717_s_153	9516479	2 Western blot analysis using specific antibodies revealed that the Grb7 SH2 domain specifically bound erbB2 and erbB3 from lysates of control cells, presumably because of the basal phosphorylation of these erbB receptors observed in ZR-75-1 cells ( 45), but this interaction was increased significantly when lysates from heregulin-stimulated cells were used (Fig.  3 A).	bind
54110	7	7171	7	NULL	NULL	0	NULL	statement 5		binding of	is higher than					statement 1		binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_13_7717_s_153	9516479	2 Western blot analysis using specific antibodies revealed that the Grb7 SH2 domain specifically bound erbB2 and erbB3 from lysates of control cells, presumably because of the basal phosphorylation of these erbB receptors observed in ZR-75-1 cells ( 45), but this interaction was increased significantly when lysates from heregulin-stimulated cells were used (Fig.  3 A).	bind
54111	8	7171	7	NULL	NULL	0	NULL	statement 6		binding of	is higher than					statement 2		binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_13_7717_s_153	9516479	2 Western blot analysis using specific antibodies revealed that the Grb7 SH2 domain specifically bound erbB2 and erbB3 from lysates of control cells, presumably because of the basal phosphorylation of these erbB receptors observed in ZR-75-1 cells ( 45), but this interaction was increased significantly when lysates from heregulin-stimulated cells were used (Fig.  3 A).	bind
22915	1	7172	6	13	NULL	NULL	NULL	Elongin C	GP	mutant	does not bind			Ala92-94		VHL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_43_27444_s_103	9341197	2 When the same Elongin C alanine-scanning mutants were tested for their abilities to bind the VHL protein using the TSK DEAE-NPR binding assay, we observed that the Elongin C mutants defective in VHL binding (C(Ala92-94), C(Ala104-105), and C(Ala110-112)) were a subset of those Elongin C alanine-scanning mutants shown previously to be defective in activation of Elongin A; we identified no Elongin C mutations that interfered with VHL binding but not the activation of Elongin A.	bind
22916	2	7172	6	13	NULL	NULL	NULL	elongin C	GP	mutant	does not bind			Ala104-105		VHL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_43_27444_s_103	9341197	2 When the same Elongin C alanine-scanning mutants were tested for their abilities to bind the VHL protein using the TSK DEAE-NPR binding assay, we observed that the Elongin C mutants defective in VHL binding (C(Ala92-94), C(Ala104-105), and C(Ala110-112)) were a subset of those Elongin C alanine-scanning mutants shown previously to be defective in activation of Elongin A; we identified no Elongin C mutations that interfered with VHL binding but not the activation of Elongin A.	bind
22917	3	7172	6	13	NULL	NULL	NULL	Elongin C	GP	mutant	does not bind			Ala110-112		VHL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_43_27444_s_103	9341197	2 When the same Elongin C alanine-scanning mutants were tested for their abilities to bind the VHL protein using the TSK DEAE-NPR binding assay, we observed that the Elongin C mutants defective in VHL binding (C(Ala92-94), C(Ala104-105), and C(Ala110-112)) were a subset of those Elongin C alanine-scanning mutants shown previously to be defective in activation of Elongin A; we identified no Elongin C mutations that interfered with VHL binding but not the activation of Elongin A.	bind
22918	4	7172	6	13	NULL	NULL	NULL	Elongin C	GP	mutant	is defective in			Ala92-94		elongin A	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_43_27444_s_103	9341197	2 When the same Elongin C alanine-scanning mutants were tested for their abilities to bind the VHL protein using the TSK DEAE-NPR binding assay, we observed that the Elongin C mutants defective in VHL binding (C(Ala92-94), C(Ala104-105), and C(Ala110-112)) were a subset of those Elongin C alanine-scanning mutants shown previously to be defective in activation of Elongin A; we identified no Elongin C mutations that interfered with VHL binding but not the activation of Elongin A.	bind
22919	5	7172	6	13	NULL	NULL	NULL	Elongin C	GP	mutant	is defective in			Ala104-105		elongin A	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_43_27444_s_103	9341197	2 When the same Elongin C alanine-scanning mutants were tested for their abilities to bind the VHL protein using the TSK DEAE-NPR binding assay, we observed that the Elongin C mutants defective in VHL binding (C(Ala92-94), C(Ala104-105), and C(Ala110-112)) were a subset of those Elongin C alanine-scanning mutants shown previously to be defective in activation of Elongin A; we identified no Elongin C mutations that interfered with VHL binding but not the activation of Elongin A.	bind
22920	6	7172	6	13	NULL	NULL	NULL	Elongin C	GP	mutant	is defective in			Ala110-112		elongin A	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_43_27444_s_103	9341197	2 When the same Elongin C alanine-scanning mutants were tested for their abilities to bind the VHL protein using the TSK DEAE-NPR binding assay, we observed that the Elongin C mutants defective in VHL binding (C(Ala92-94), C(Ala104-105), and C(Ala110-112)) were a subset of those Elongin C alanine-scanning mutants shown previously to be defective in activation of Elongin A; we identified no Elongin C mutations that interfered with VHL binding but not the activation of Elongin A.	bind
27860	1	7172	7	NULL	NULL	0	NULL	Elongin C	NULL	mutant	does not bind	NULL		C(Ala92-94)		VHL	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_43_27444_s_103	9341197	2 When the same Elongin C alanine-scanning mutants were tested for their abilities to bind the VHL protein using the TSK DEAE-NPR binding assay, we observed that the Elongin C mutants defective in VHL binding (C(Ala92-94), C(Ala104-105), and C(Ala110-112)) were a subset of those Elongin C alanine-scanning mutants shown previously to be defective in activation of Elongin A; we identified no Elongin C mutations that interfered with VHL binding but not the activation of Elongin A.	bind
27861	2	7172	7	NULL	NULL	0	NULL	Elongin C	NULL	mutant	does not bind	NULL		C(Ala104-105)		VHL	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_43_27444_s_103	9341197	2 When the same Elongin C alanine-scanning mutants were tested for their abilities to bind the VHL protein using the TSK DEAE-NPR binding assay, we observed that the Elongin C mutants defective in VHL binding (C(Ala92-94), C(Ala104-105), and C(Ala110-112)) were a subset of those Elongin C alanine-scanning mutants shown previously to be defective in activation of Elongin A; we identified no Elongin C mutations that interfered with VHL binding but not the activation of Elongin A.	bind
27862	3	7172	7	NULL	NULL	0	NULL	Elongin C	NULL	mutant	does not bind	NULL		C(Ala110-112)		VHL	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_43_27444_s_103	9341197	2 When the same Elongin C alanine-scanning mutants were tested for their abilities to bind the VHL protein using the TSK DEAE-NPR binding assay, we observed that the Elongin C mutants defective in VHL binding (C(Ala92-94), C(Ala104-105), and C(Ala110-112)) were a subset of those Elongin C alanine-scanning mutants shown previously to be defective in activation of Elongin A; we identified no Elongin C mutations that interfered with VHL binding but not the activation of Elongin A.	bind
27863	4	7172	7	NULL	NULL	0	NULL	Elongin C	NULL	mutant	does not activate	NULL		C(Ala92-94)		Elongin A	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_43_27444_s_103	9341197	2 When the same Elongin C alanine-scanning mutants were tested for their abilities to bind the VHL protein using the TSK DEAE-NPR binding assay, we observed that the Elongin C mutants defective in VHL binding (C(Ala92-94), C(Ala104-105), and C(Ala110-112)) were a subset of those Elongin C alanine-scanning mutants shown previously to be defective in activation of Elongin A; we identified no Elongin C mutations that interfered with VHL binding but not the activation of Elongin A.	bind
27864	5	7172	7	NULL	NULL	0	NULL	Elongin C	NULL	mutant	does not activate	NULL		C(Ala104-105)		Elongin A	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_43_27444_s_103	9341197	2 When the same Elongin C alanine-scanning mutants were tested for their abilities to bind the VHL protein using the TSK DEAE-NPR binding assay, we observed that the Elongin C mutants defective in VHL binding (C(Ala92-94), C(Ala104-105), and C(Ala110-112)) were a subset of those Elongin C alanine-scanning mutants shown previously to be defective in activation of Elongin A; we identified no Elongin C mutations that interfered with VHL binding but not the activation of Elongin A.	bind
27865	6	7172	7	NULL	NULL	0	NULL	Elongin C	NULL	mutant	does not activate	NULL		C(Ala110-112)		Elongin A	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_43_27444_s_103	9341197	2 When the same Elongin C alanine-scanning mutants were tested for their abilities to bind the VHL protein using the TSK DEAE-NPR binding assay, we observed that the Elongin C mutants defective in VHL binding (C(Ala92-94), C(Ala104-105), and C(Ala110-112)) were a subset of those Elongin C alanine-scanning mutants shown previously to be defective in activation of Elongin A; we identified no Elongin C mutations that interfered with VHL binding but not the activation of Elongin A.	bind
22547	1	7173	6	13	NULL	NULL	NULL	TRAF2	GP		bind					T2bs-C	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_31572_s_270	16020544	2 Whereas this indicates that Etk/mx is not the intermediary protein for the binding of TRAF2 to T2bs-C, the fact that Etk/mx can bind to T2bs-C indicates that TRAF2 may be indirectly recruited to T2bs-C by a protein with homology to Etk/Bmx.	bind
22548	2	7173	6	13	NULL	NULL	NULL	Etk/mx	GP		bind					T2bs-C	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_31572_s_270	16020544	2 Whereas this indicates that Etk/mx is not the intermediary protein for the binding of TRAF2 to T2bs-C, the fact that Etk/mx can bind to T2bs-C indicates that TRAF2 may be indirectly recruited to T2bs-C by a protein with homology to Etk/Bmx.	bind
22582	3	7173	6	13	NULL	NULL	NULL	TRAF2	GP		is recruited to		indirectly			T2bs-C	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_31572_s_270	16020544	2 Whereas this indicates that Etk/mx is not the intermediary protein for the binding of TRAF2 to T2bs-C, the fact that Etk/mx can bind to T2bs-C indicates that TRAF2 may be indirectly recruited to T2bs-C by a protein with homology to Etk/Bmx.	bind
22583	4	7173	6	13	NULL	NULL	NULL	statement 3	Process		occurs by					Etk/Bmx homologous protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_31572_s_270	16020544	2 Whereas this indicates that Etk/mx is not the intermediary protein for the binding of TRAF2 to T2bs-C, the fact that Etk/mx can bind to T2bs-C indicates that TRAF2 may be indirectly recruited to T2bs-C by a protein with homology to Etk/Bmx.	bind
26957	1	7173	7	NULL	NULL	0	NULL	 TRAF2 	NULL		bind	NULL				 T2bs-C	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_36_31572_s_270	16020544	2 Whereas this indicates that Etk/mx is not the intermediary protein for the binding of TRAF2 to T2bs-C, the fact that Etk/mx can bind to T2bs-C indicates that TRAF2 may be indirectly recruited to T2bs-C by a protein with homology to Etk/Bmx.	bind
26958	2	7173	7	NULL	NULL	0	NULL	Etk/mx	NULL		bind	NULL				T2bs-C 	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_36_31572_s_270	16020544	2 Whereas this indicates that Etk/mx is not the intermediary protein for the binding of TRAF2 to T2bs-C, the fact that Etk/mx can bind to T2bs-C indicates that TRAF2 may be indirectly recruited to T2bs-C by a protein with homology to Etk/Bmx.	bind
26959	3	7173	7	NULL	NULL	0	NULL	 TRAF2	NULL		recruited to	NULL	indirectly			T2bs-C	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_36_31572_s_270	16020544	2 Whereas this indicates that Etk/mx is not the intermediary protein for the binding of TRAF2 to T2bs-C, the fact that Etk/mx can bind to T2bs-C indicates that TRAF2 may be indirectly recruited to T2bs-C by a protein with homology to Etk/Bmx.	bind
26960	4	7173	7	NULL	NULL	0	NULL	statement 3	NULL		occurs by a	NULL				Etk/Bmx homologous protein	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_31572_s_270	16020544	2 Whereas this indicates that Etk/mx is not the intermediary protein for the binding of TRAF2 to T2bs-C, the fact that Etk/mx can bind to T2bs-C indicates that TRAF2 may be indirectly recruited to T2bs-C by a protein with homology to Etk/Bmx.	bind
26961	5	7173	7	NULL	NULL	0	NULL	Etk/mx	NULL		is not an	NULL				intermediary protein	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_31572_s_270	16020544	2 Whereas this indicates that Etk/mx is not the intermediary protein for the binding of TRAF2 to T2bs-C, the fact that Etk/mx can bind to T2bs-C indicates that TRAF2 may be indirectly recruited to T2bs-C by a protein with homology to Etk/Bmx.	bind
37600	6	7173	7	NULL	NULL	0	NULL	statement 1	NULL		does not occur through	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_36_31572_s_270	16020544	2 Whereas this indicates that Etk/mx is not the intermediary protein for the binding of TRAF2 to T2bs-C, the fact that Etk/mx can bind to T2bs-C indicates that TRAF2 may be indirectly recruited to T2bs-C by a protein with homology to Etk/Bmx.	bind
22584	1	7174	6	13	NULL	NULL	NULL	CD36	GP		expressed in					COS cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_41_26338_s_128	9756864	2 While this manuscript was in preparation, Calvo  et al. ( 64) reported their independent observation that HDL binds to CD36 expressed in COS and Sf9 cells.	bind
22585	2	7174	6	13	NULL	NULL	NULL	CD36	GP		expressed in					Sf9 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_41_26338_s_128	9756864	2 While this manuscript was in preparation, Calvo  et al. ( 64) reported their independent observation that HDL binds to CD36 expressed in COS and Sf9 cells.	bind
22586	3	7174	6	13	NULL	NULL	NULL	HDL	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_41_26338_s_128	9756864	2 While this manuscript was in preparation, Calvo  et al. ( 64) reported their independent observation that HDL binds to CD36 expressed in COS and Sf9 cells.	bind
22587	4	7174	6	13	NULL	NULL	NULL	HDL	GP		bind					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_41_26338_s_128	9756864	2 While this manuscript was in preparation, Calvo  et al. ( 64) reported their independent observation that HDL binds to CD36 expressed in COS and Sf9 cells.	bind
26962	2	7174	7	NULL	NULL	0	NULL	HDL	NULL		binds to	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_41_26338_s_128	9756864	2 While this manuscript was in preparation, Calvo  et al. ( 64) reported their independent observation that HDL binds to CD36 expressed in COS and Sf9 cells.	bind
26963	1	7174	7	NULL	NULL	0	NULL	CD36	NULL		expressed in	NULL				COS cells	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_41_26338_s_128	9756864	2 While this manuscript was in preparation, Calvo  et al. ( 64) reported their independent observation that HDL binds to CD36 expressed in COS and Sf9 cells.	bind
37601	3	7174	7	NULL	NULL	0	NULL	CD36	NULL		expressed in	NULL				Sf9 cells	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_41_26338_s_128	9756864	2 While this manuscript was in preparation, Calvo  et al. ( 64) reported their independent observation that HDL binds to CD36 expressed in COS and Sf9 cells.	bind
37602	4	7174	7	NULL	NULL	0	NULL	HDL	NULL		binds to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_41_26338_s_128	9756864	2 While this manuscript was in preparation, Calvo  et al. ( 64) reported their independent observation that HDL binds to CD36 expressed in COS and Sf9 cells.	bind
22588	1	7175	6	13	NULL	NULL	NULL	DnaA protein	GP		bind					dnaA	G			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_37_23017_s_18	9287298	2 With an  in vivo assay that measured the binding of DnaA protein to the  dnaA promoter region of a  dnaA promoter- lacZ fusion, encoding amino acid substitutions within the C-terminal 89 residues or lacking C-terminal coding sequence were unable to repress expression.	bind
26964	1	7175	7	10	NULL	0	NULL	DnaA protein	NULL		bind	NULL				dnaA	NULL			promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_37_23017_s_18	9287298	2 With an  in vivo assay that measured the binding of DnaA protein to the  dnaA promoter region of a  dnaA promoter- lacZ fusion, encoding amino acid substitutions within the C-terminal 89 residues or lacking C-terminal coding sequence were unable to repress expression.	bind
22589	1	7176	6	13	NULL	NULL	NULL	secYEG	GP		bind					SecA	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_14_13769_s_211	14722060	2 With the experimentally determined  koff value (4 x 10-3 s-1), the apparent  Kd values for MANT-ADP and MANT-ATP binding to the SecYEG-bound SecA correspond to 21 and 59 nM, respectively.	bind
22590	2	7176	6	13	NULL	NULL	NULL	mant-ADP	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_14_13769_s_211	14722060	2 With the experimentally determined  koff value (4 x 10-3 s-1), the apparent  Kd values for MANT-ADP and MANT-ATP binding to the SecYEG-bound SecA correspond to 21 and 59 nM, respectively.	bind
22591	3	7176	6	13	NULL	NULL	NULL	mant-ATP	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_14_13769_s_211	14722060	2 With the experimentally determined  koff value (4 x 10-3 s-1), the apparent  Kd values for MANT-ADP and MANT-ATP binding to the SecYEG-bound SecA correspond to 21 and 59 nM, respectively.	bind
26965	2	7176	7	10	NULL	0	NULL	MANT-ADP	NULL		bind	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_14_13769_s_211	14722060	2 With the experimentally determined  koff value (4 x 10-3 s-1), the apparent  Kd values for MANT-ADP and MANT-ATP binding to the SecYEG-bound SecA correspond to 21 and 59 nM, respectively.	bind
26966	3	7176	7	10	NULL	0	NULL	MANT-ATP	NULL		bind	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_14_13769_s_211	14722060	2 With the experimentally determined  koff value (4 x 10-3 s-1), the apparent  Kd values for MANT-ADP and MANT-ATP binding to the SecYEG-bound SecA correspond to 21 and 59 nM, respectively.	bind
46455	1	7176	7	10	NULL	0	NULL	SecYEG	NULL		bind	NULL				SecA	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_14_13769_s_211	14722060	2 With the experimentally determined  koff value (4 x 10-3 s-1), the apparent  Kd values for MANT-ADP and MANT-ATP binding to the SecYEG-bound SecA correspond to 21 and 59 nM, respectively.	bind
22592	1	7177	6	13	NULL	NULL	NULL				bind			RCC1-like domains		GTP-binding proteins	GP	small			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_20_12148_s_212	9575161	2 WW domains have been implicated in the binding of peptides containing PY and PY-like domains (Ref.  32, and references therein), and it is suggested that RCC1-like domains bind small GTP-binding proteins ( 23).	bind
22593	2	7177	6	13	NULL	NULL	NULL				plays a role in			WW domain		peptides 	GP	binding of	PY domain		NULL	 	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_20_12148_s_212	9575161	2 WW domains have been implicated in the binding of peptides containing PY and PY-like domains (Ref.  32, and references therein), and it is suggested that RCC1-like domains bind small GTP-binding proteins ( 23).	bind
22594	3	7177	6	13	NULL	NULL	NULL				plays a role in			WW domain		peptides	GP	binding of	PY-like domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_20_12148_s_212	9575161	2 WW domains have been implicated in the binding of peptides containing PY and PY-like domains (Ref.  32, and references therein), and it is suggested that RCC1-like domains bind small GTP-binding proteins ( 23).	bind
26967	1	7177	7	10	NULL	0	NULL		NULL		plays a role in	NULL		 WW domains		peptides	NULL	binding of	PY domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_20_12148_s_212	9575161	2 WW domains have been implicated in the binding of peptides containing PY and PY-like domains (Ref.  32, and references therein), and it is suggested that RCC1-like domains bind small GTP-binding proteins ( 23).	bind
26968	2	7177	7	10	NULL	0	NULL		NULL		plays a role in	NULL		WW domains		peptides	NULL	binding of	PY-like domains		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_20_12148_s_212	9575161	2 WW domains have been implicated in the binding of peptides containing PY and PY-like domains (Ref.  32, and references therein), and it is suggested that RCC1-like domains bind small GTP-binding proteins ( 23).	bind
26969	3	7177	7	NULL	NULL	0	NULL		NULL		bind	NULL		RCC1-like domains		GTP-binding proteins	NULL	small			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_20_12148_s_212	9575161	2 WW domains have been implicated in the binding of peptides containing PY and PY-like domains (Ref.  32, and references therein), and it is suggested that RCC1-like domains bind small GTP-binding proteins ( 23).	bind
22595	1	7179	6	13	NULL	NULL	NULL	EF	GP		bind					AC toxins	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_19_19955_s_50	14981084	2''-d-3''-ANT-ATP fluorescence increases upon binding of the EF and ACT activator calmodulin to the AC toxins ( ,  ).	bind
22596	2	7179	6	13	NULL	NULL	NULL	calmodulin	GP		bind					AC toxins	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_19_19955_s_50	14981084	2''-d-3''-ANT-ATP fluorescence increases upon binding of the EF and ACT activator calmodulin to the AC toxins ( ,  ).	bind
46456	3	7179	6	13	NULL	NULL	NULL	calmodulin	GP		is a type of					ACT activator	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_19_19955_s_50	14981084	2''-d-3''-ANT-ATP fluorescence increases upon binding of the EF and ACT activator calmodulin to the AC toxins ( ,  ).	bind
26970	1	7179	7	NULL	NULL	0	NULL	EF	NULL		bind	NULL				AC toxins	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_19_19955_s_50	14981084	2''-d-3''-ANT-ATP fluorescence increases upon binding of the EF and ACT activator calmodulin to the AC toxins ( ,  ).	bind
26971	2	7179	7	NULL	NULL	0	NULL	calmodulin	NULL		bind	NULL				AC toxins	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_19_19955_s_50	14981084	2''-d-3''-ANT-ATP fluorescence increases upon binding of the EF and ACT activator calmodulin to the AC toxins ( ,  ).	bind
26972	3	7179	7	NULL	NULL	0	NULL	calmodulin	NULL		is a type of	NULL				ACT activator	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_19_19955_s_50	14981084	2''-d-3''-ANT-ATP fluorescence increases upon binding of the EF and ACT activator calmodulin to the AC toxins ( ,  ).	bind
22597	1	7180	6	13	NULL	NULL	NULL	mammalian membrane	CellComponent		bind					AC	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_12_11513_s_153	15649897	2''-substituted nucleotides and nucleosides also inhibit mammalian membrane-bound AC in a mixed competitive manner ( ).	bind
22598	2	7180	6	13	NULL	NULL	NULL	nucleotides	NucleicAcid	substituted	bind					AC	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_12_11513_s_153	15649897	2''-substituted nucleotides and nucleosides also inhibit mammalian membrane-bound AC in a mixed competitive manner ( ).	bind
22599	3	7180	6	13	NULL	NULL	NULL	nucleosides	GP	substituted	bind					AC	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_12_11513_s_153	15649897	2''-substituted nucleotides and nucleosides also inhibit mammalian membrane-bound AC in a mixed competitive manner ( ).	bind
22600	4	7180	6	13	NULL	NULL	NULL	statement 2	Process		inhibit		competitively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_12_11513_s_153	15649897	2''-substituted nucleotides and nucleosides also inhibit mammalian membrane-bound AC in a mixed competitive manner ( ).	bind
22601	5	7180	6	13	NULL	NULL	NULL	statement 3	Process		inhibit		competitively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_12_11513_s_153	15649897	2''-substituted nucleotides and nucleosides also inhibit mammalian membrane-bound AC in a mixed competitive manner ( ).	bind
26975	2	7180	7	10	NULL	0	NULL	nucleotides	NULL	2''-substituted	bind	NULL				AC	NULL	 			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_12_11513_s_153	15649897	2''-substituted nucleotides and nucleosides also inhibit mammalian membrane-bound AC in a mixed competitive manner ( ).	bind
26976	3	7180	7	10	NULL	0	NULL	nucleosides 	NULL	2''-substituted	bind	NULL				AC	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_12_11513_s_153	15649897	2''-substituted nucleotides and nucleosides also inhibit mammalian membrane-bound AC in a mixed competitive manner ( ).	bind
37619	1	7180	7	NULL	NULL	0	NULL	mammalian membrane	NULL		bind	NULL				AC	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_12_11513_s_153	15649897	2''-substituted nucleotides and nucleosides also inhibit mammalian membrane-bound AC in a mixed competitive manner ( ).	bind
37620	4	7180	7	NULL	NULL	0	NULL	statement 2	NULL		inhibit	NULL	competitively			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_12_11513_s_153	15649897	2''-substituted nucleotides and nucleosides also inhibit mammalian membrane-bound AC in a mixed competitive manner ( ).	bind
37621	5	7180	7	NULL	NULL	0	NULL	statement 3	NULL		inhibit	NULL	competitively			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_12_11513_s_153	15649897	2''-substituted nucleotides and nucleosides also inhibit mammalian membrane-bound AC in a mixed competitive manner ( ).	bind
22602	1	7181	6	13	NULL	NULL	NULL	GTPgamma35S	GP		bind					Galphaq	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_55_2_339_s_274	9927627	2) A marked degree of constitutive activity is detectable for both the A293E and D142A mutants also in a membrane assay (in which desensitization should not occur) measuring receptor-mediated stimulation of GTPgamma35S binding to Galphaq (our unpublished results).	bind
22603	2	7181	6	13	NULL	NULL	NULL	statement 1	Process	stimulation of	is mediated through					receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_55_2_339_s_274	9927627	2) A marked degree of constitutive activity is detectable for both the A293E and D142A mutants also in a membrane assay (in which desensitization should not occur) measuring receptor-mediated stimulation of GTPgamma35S binding to Galphaq (our unpublished results).	bind
26977	1	7181	7	NULL	NULL	0	NULL	GTPgamma35S	NULL		bind	NULL				Galphaq	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_55_2_339_s_274	9927627	2) A marked degree of constitutive activity is detectable for both the A293E and D142A mutants also in a membrane assay (in which desensitization should not occur) measuring receptor-mediated stimulation of GTPgamma35S binding to Galphaq (our unpublished results).	bind
26978	2	7181	7	NULL	NULL	0	NULL	receptor	NULL		mediates	NULL				statement 1	NULL	stimulation of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_55_2_339_s_274	9927627	2) A marked degree of constitutive activity is detectable for both the A293E and D142A mutants also in a membrane assay (in which desensitization should not occur) measuring receptor-mediated stimulation of GTPgamma35S binding to Galphaq (our unpublished results).	bind
22604	1	7182	6	13	NULL	NULL	NULL	S3 dimer	GP		bind					LPS micelle	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_48_50150_s_276	15328339	2) At the initial low ratio of S3:LPS, binding of the S3 dimer to LPS micelle occurs via electrostatic and hydrophobic interactions.	bind
22605	2	7182	6	13	NULL	NULL	NULL	statement 1	Process		occurs via					electrostatic interactions	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_48_50150_s_276	15328339	2) At the initial low ratio of S3:LPS, binding of the S3 dimer to LPS micelle occurs via electrostatic and hydrophobic interactions.	bind
22606	3	7182	6	13	NULL	NULL	NULL	statement 1	Process		occurs via					hydrophobic interactions	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_48_50150_s_276	15328339	2) At the initial low ratio of S3:LPS, binding of the S3 dimer to LPS micelle occurs via electrostatic and hydrophobic interactions.	bind
26979	1	7182	7	NULL	NULL	0	NULL	 S3 dimer	NULL		bind	NULL				LPS micelle	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_50150_s_276	15328339	2) At the initial low ratio of S3:LPS, binding of the S3 dimer to LPS micelle occurs via electrostatic and hydrophobic interactions.	bind
26980	2	7182	7	NULL	NULL	0	NULL	statement 1	NULL		occurs via	NULL				electrostatic interaction	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_50150_s_276	15328339	2) At the initial low ratio of S3:LPS, binding of the S3 dimer to LPS micelle occurs via electrostatic and hydrophobic interactions.	bind
26981	3	7182	7	NULL	NULL	0	NULL	statement 1	NULL		occurs via	NULL				hydrophobic interaction	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_48_50150_s_276	15328339	2) At the initial low ratio of S3:LPS, binding of the S3 dimer to LPS micelle occurs via electrostatic and hydrophobic interactions.	bind
22607	1	7183	6	13	NULL	NULL	NULL	NCoR	GP		bind					TR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_46_30175_s_225	9804773	2) Both NCoR and SRC-1 do not bind simultaneously to TR, suggesting at least two discreet steps are necessary for transactivation.	bind
22608	2	7183	6	13	NULL	NULL	NULL	SRC-1	GP		bind					TR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_46_30175_s_225	9804773	2) Both NCoR and SRC-1 do not bind simultaneously to TR, suggesting at least two discreet steps are necessary for transactivation.	bind
22609	3	7183	6	13	NULL	NULL	NULL	statement 1	Process		does not occur simultaneously with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_46_30175_s_225	9804773	2) Both NCoR and SRC-1 do not bind simultaneously to TR, suggesting at least two discreet steps are necessary for transactivation.	bind
26982	1	7183	7	NULL	NULL	0	NULL	NCoR	NULL		bind	NULL				TR	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_46_30175_s_225	9804773	2) Both NCoR and SRC-1 do not bind simultaneously to TR, suggesting at least two discreet steps are necessary for transactivation.	bind
26983	2	7183	7	NULL	NULL	0	NULL	SRC-1	NULL		 bind	NULL				TR	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_46_30175_s_225	9804773	2) Both NCoR and SRC-1 do not bind simultaneously to TR, suggesting at least two discreet steps are necessary for transactivation.	bind
37622	3	7183	7	NULL	NULL	0	NULL	statement 1	NULL		does not occur simulataneous with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_46_30175_s_225	9804773	2) Both NCoR and SRC-1 do not bind simultaneously to TR, suggesting at least two discreet steps are necessary for transactivation.	bind
22610	1	7184	6	13	NULL	NULL	NULL	BRMS1	GP		bind			delta204-246		HDAC1.RpAp46/48	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
22611	2	7184	6	13	NULL	NULL	NULL	BRMS1	GP	full length	bind					HDAC1.RpAp46/48	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
22612	3	7184	6	13	NULL	NULL	NULL	statement 1	Process		is less than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
22613	4	7184	6	13	NULL	NULL	NULL	BRMS1	GP		bind			delta204-246		mSin3A	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
22614	5	7184	6	13	NULL	NULL	NULL	BRMS1	GP		bind			delta204-246		mSin3B	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
22615	6	7184	6	13	NULL	NULL	NULL	BRMS1	GP		bind			delta204-246		SAP30	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
22616	7	7184	6	13	NULL	NULL	NULL	BRMS1	GP		bind			delta204-246		HDAC2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
22617	8	7184	6	13	NULL	NULL	NULL	BRMS1	GP		bind			delta204-246		RBP1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
22618	9	7184	6	13	NULL	NULL	NULL	BRMS1	GP	full length	bind					mSin3A	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
22619	10	7184	6	13	NULL	NULL	NULL	BRMS1	GP	full length	bind					mSin3B	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
22620	11	7184	6	13	NULL	NULL	NULL	BRMS1	GP	full length	bind					SAP30	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
22621	12	7184	6	13	NULL	NULL	NULL	BRMS1	GP	full length	bind					RBP1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
22622	13	7184	6	13	NULL	NULL	NULL	BRMS1	GP	full length	bind					HDAC2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
22623	14	7184	6	13	NULL	NULL	NULL	statement 4	Process		is as effective as					statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
22624	15	7184	6	13	NULL	NULL	NULL	statement 5	Process		is as effective as					statement 10	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
22625	16	7184	6	13	NULL	NULL	NULL	statement 6	Process		is as effective as					statement 11	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
22626	17	7184	6	13	NULL	NULL	NULL	statement 7	Process		is as effective as					statement 13	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
22627	18	7184	6	13	NULL	NULL	NULL	statement 8	Process		is as effective as					statement 12	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
26984	1	7184	7	NULL	NULL	0	NULL	BRMS1	NULL		bind	NULL	less effectively	delta204-246		HDAC1.RpAp46/48	NULL		core subunit		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
26985	2	7184	7	NULL	NULL	0	NULL	BRMS1	NULL	full-length	bind	NULL				HDAC1.RpAp46/48	NULL		core subunit		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
26986	3	7184	7	10	NULL	0	NULL	statement 1	NULL		is less than	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
26987	4	7184	7	NULL	NULL	0	NULL	BRMS1	NULL		binds	NULL		delta204-246		mSin3A	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
26988	5	7184	7	NULL	NULL	0	NULL	BRMS1	NULL		binds	NULL		delta204-246		mSin3B	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
26989	6	7184	7	NULL	NULL	0	NULL	BRMS1	NULL		binds	NULL		delta204-246		SAP30	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
26990	7	7184	7	NULL	NULL	0	NULL	BRMS1	NULL		binds 	NULL		delta204-246		HDAC2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
26991	8	7184	7	NULL	NULL	0	NULL	BRMS1	NULL		binds	NULL		delta204-246		RBP1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
37623	9	7184	7	NULL	NULL	0	NULL	BRMS1	NULL	full-length	binds	NULL				mSin3A	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
37625	10	7184	7	NULL	NULL	0	NULL	statement 4	NULL		is as effective as	NULL				statement 9	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
37626	11	7184	7	NULL	NULL	0	NULL	BRMS1	NULL	full-length	bind	NULL				mSin3B	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
37627	12	7184	7	NULL	NULL	0	NULL	statement 5	NULL		is as effective as	NULL				statement 11	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
37628	13	7184	7	NULL	NULL	0	NULL	BRMS1	NULL	full-length	bind	NULL				SAP30	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
37629	14	7184	7	NULL	NULL	0	NULL	statement 6	NULL		is as effective as	NULL				statement 13	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
37630	15	7184	7	NULL	NULL	0	NULL	BRMS1	NULL	full-length	bind	NULL				HDAC2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
37631	16	7184	7	NULL	NULL	0	NULL	statement 7	NULL		is as effective as	NULL				statement 15	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
37632	17	7184	7	NULL	NULL	0	NULL	BRMS1	NULL	full-length	bind	NULL				RBP1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
37633	18	7184	7	NULL	NULL	0	NULL	statement 8	NULL		is as effective as	NULL				statement 17	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_2_1562_s_312	14581478	2) BRMS1 has distinct binding site(s) for the HDAC1.RbAp46/48 core subunit as compared with the rest of the complex (mSin3A, mSin3B, SAP30, HDAC2, and RBP1) as demonstrated by BRMS1(delta204-246) binding less effectively to HDAC1.RpAp46/48 than does full-length BRMS1; in contrast, BRMS1(delta204-246) binds the remaining complex components as effectively ( Fig. 4).	bind
22628	1	7186	6	13	NULL	NULL	NULL				bind			Domain Ia		LRP/alpha2MR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_11_7566_s_39	10713063	2) Domain Ia binds to LRP/alpha2MR and is internalized via endosomes to the transreticular Golgi ( 27).	bind
22629	2	7186	6	13	NULL	NULL	NULL				is internalized to			Domain Ia		transreticular Golgi	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_11_7566_s_39	10713063	2) Domain Ia binds to LRP/alpha2MR and is internalized via endosomes to the transreticular Golgi ( 27).	bind
22630	3	7186	6	13	NULL	NULL	NULL	statement 2	Process		occurs via					endosomes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_11_7566_s_39	10713063	2) Domain Ia binds to LRP/alpha2MR and is internalized via endosomes to the transreticular Golgi ( 27).	bind
26994	1	7186	7	NULL	NULL	0	NULL		NULL		bind	NULL		Domain Ia 		LRP/alpha2MR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_11_7566_s_39	10713063	2) Domain Ia binds to LRP/alpha2MR and is internalized via endosomes to the transreticular Golgi ( 27).	bind
26995	2	7186	7	NULL	NULL	0	NULL		NULL		is internalized to	NULL		Domain Ia 		transreticular Golgi	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_11_7566_s_39	10713063	2) Domain Ia binds to LRP/alpha2MR and is internalized via endosomes to the transreticular Golgi ( 27).	bind
26996	3	7186	7	NULL	NULL	0	NULL	statement 2	NULL		occurs via	NULL				endosomes	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_11_7566_s_39	10713063	2) Domain Ia binds to LRP/alpha2MR and is internalized via endosomes to the transreticular Golgi ( 27).	bind
22631	1	7187	6	13	NULL	NULL	NULL	E2F	GP		bind					DHFR-E2F oligonucleotide	NucleicAcid	hamster			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_2_1218_s_211	8557653	2) E2F binds to the hamster DHFR-E2F  oligonucleotide only in the presence of salmon sperm DNA but not with  poly(dI-dC) as carrier DNA ( Fig. 7,  lanes 7- 11).	bind
22632	2	7187	6	13	NULL	NULL	NULL	statement 1	Process		occurs in presence of		only			sperm DNA	NucleicAcid	salmon			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_2_1218_s_211	8557653	2) E2F binds to the hamster DHFR-E2F  oligonucleotide only in the presence of salmon sperm DNA but not with  poly(dI-dC) as carrier DNA ( Fig. 7,  lanes 7- 11).	bind
22633	3	7187	6	13	NULL	NULL	NULL	statement 1	Process		occurs in absence of					poly(dI-dC)	NucleicAcid	carrier DNA			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_2_1218_s_211	8557653	2) E2F binds to the hamster DHFR-E2F  oligonucleotide only in the presence of salmon sperm DNA but not with  poly(dI-dC) as carrier DNA ( Fig. 7,  lanes 7- 11).	bind
26997	1	7187	7	NULL	NULL	0	NULL	 E2F	NULL		binds to	NULL				DHFR-E2F oligonucleotide	NULL	hamster			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_2_1218_s_211	8557653	2) E2F binds to the hamster DHFR-E2F  oligonucleotide only in the presence of salmon sperm DNA but not with  poly(dI-dC) as carrier DNA ( Fig. 7,  lanes 7- 11).	bind
26998	2	7187	7	NULL	NULL	0	NULL	statement 1	NULL		in presence of	NULL				sperm DNA	NULL	salmon			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_2_1218_s_211	8557653	2) E2F binds to the hamster DHFR-E2F  oligonucleotide only in the presence of salmon sperm DNA but not with  poly(dI-dC) as carrier DNA ( Fig. 7,  lanes 7- 11).	bind
26999	3	7187	7	NULL	NULL	0	NULL	statement 1	NULL		does not occur with	NULL				poly(dI-dC)	NULL	carrier DNA			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_2_1218_s_211	8557653	2) E2F binds to the hamster DHFR-E2F  oligonucleotide only in the presence of salmon sperm DNA but not with  poly(dI-dC) as carrier DNA ( Fig. 7,  lanes 7- 11).	bind
22663	1	7188	6	13	NULL	NULL	NULL	iNOS	GP		encompasses				promoter					HIF-1 binding site	NULL	ANA-1 macrophages	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_18_12236_s_178	9115299	2) encompassing the HIF-1 binding site of the iNOS promoter in ANA-1 macrophages.	bind
27000	1	7188	7	NULL	NULL	0	NULL	 iNOS	NULL		contains	NULL			promoter		NULL			HIF-1 binding site	NULL	ANA-1 macrophages	0	NULL	NULL	NULL	gw60_jbiolchem_272_18_12236_s_178	9115299	2) encompassing the HIF-1 binding site of the iNOS promoter in ANA-1 macrophages.	bind
22664	1	7189	6	13	NULL	NULL	NULL	FGF-2	GP		bind		directly			TSP	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_8_12_2449_s_37	9398667	2) FGF-2 binds directly to TSP (Taraboletti  et al., 1997  ) and may interact also with other adhesive proteins including FN, laminin, and collagen (Feige  et al., 1989  ).	bind
22665	2	7189	6	13	NULL	NULL	NULL	FGF-2	GP		interact with		may			FN	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_8_12_2449_s_37	9398667	2) FGF-2 binds directly to TSP (Taraboletti  et al., 1997  ) and may interact also with other adhesive proteins including FN, laminin, and collagen (Feige  et al., 1989  ).	bind
22666	3	7189	6	13	NULL	NULL	NULL	FGF-2	GP		interact with		may			laminin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_8_12_2449_s_37	9398667	2) FGF-2 binds directly to TSP (Taraboletti  et al., 1997  ) and may interact also with other adhesive proteins including FN, laminin, and collagen (Feige  et al., 1989  ).	bind
22667	4	7189	6	13	NULL	NULL	NULL	FGF-2	GP		interact with		may			collagen	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_8_12_2449_s_37	9398667	2) FGF-2 binds directly to TSP (Taraboletti  et al., 1997  ) and may interact also with other adhesive proteins including FN, laminin, and collagen (Feige  et al., 1989  ).	bind
37431	5	7189	6	13	NULL	NULL	NULL	FN	GP		is a type of					adhesive protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_8_12_2449_s_37	9398667	2) FGF-2 binds directly to TSP (Taraboletti  et al., 1997  ) and may interact also with other adhesive proteins including FN, laminin, and collagen (Feige  et al., 1989  ).	bind
37432	6	7189	6	13	NULL	NULL	NULL	laminin	GP		is a type of					adhesive protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_8_12_2449_s_37	9398667	2) FGF-2 binds directly to TSP (Taraboletti  et al., 1997  ) and may interact also with other adhesive proteins including FN, laminin, and collagen (Feige  et al., 1989  ).	bind
37433	7	7189	6	13	NULL	NULL	NULL	collagen	GP		is a type of					adhesive protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_8_12_2449_s_37	9398667	2) FGF-2 binds directly to TSP (Taraboletti  et al., 1997  ) and may interact also with other adhesive proteins including FN, laminin, and collagen (Feige  et al., 1989  ).	bind
27001	1	7189	7	NULL	NULL	0	NULL	FGF-2	NULL		binds	NULL	directly			TSP	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_8_12_2449_s_37	9398667	2) FGF-2 binds directly to TSP (Taraboletti  et al., 1997  ) and may interact also with other adhesive proteins including FN, laminin, and collagen (Feige  et al., 1989  ).	bind
27002	2	7189	7	NULL	NULL	0	NULL	FGF-2	NULL		interact with	NULL	may			FN	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_8_12_2449_s_37	9398667	2) FGF-2 binds directly to TSP (Taraboletti  et al., 1997  ) and may interact also with other adhesive proteins including FN, laminin, and collagen (Feige  et al., 1989  ).	bind
27003	3	7189	7	NULL	NULL	0	NULL	FGF-2	NULL		interact with	NULL	may			laminin	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_8_12_2449_s_37	9398667	2) FGF-2 binds directly to TSP (Taraboletti  et al., 1997  ) and may interact also with other adhesive proteins including FN, laminin, and collagen (Feige  et al., 1989  ).	bind
27004	4	7189	7	NULL	NULL	0	NULL	FGF-2	NULL		interact with	NULL	may			collagen	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_8_12_2449_s_37	9398667	2) FGF-2 binds directly to TSP (Taraboletti  et al., 1997  ) and may interact also with other adhesive proteins including FN, laminin, and collagen (Feige  et al., 1989  ).	bind
27005	5	7189	7	NULL	NULL	0	NULL	FN	NULL		is a type of	NULL				adhesive protein	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_8_12_2449_s_37	9398667	2) FGF-2 binds directly to TSP (Taraboletti  et al., 1997  ) and may interact also with other adhesive proteins including FN, laminin, and collagen (Feige  et al., 1989  ).	bind
27006	6	7189	7	NULL	NULL	0	NULL	laminin	NULL		is a type of	NULL				adhesive protein	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_8_12_2449_s_37	9398667	2) FGF-2 binds directly to TSP (Taraboletti  et al., 1997  ) and may interact also with other adhesive proteins including FN, laminin, and collagen (Feige  et al., 1989  ).	bind
27007	7	7189	7	NULL	NULL	0	NULL	collagen	NULL		is a type of	NULL				adhesive protein	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_8_12_2449_s_37	9398667	2) FGF-2 binds directly to TSP (Taraboletti  et al., 1997  ) and may interact also with other adhesive proteins including FN, laminin, and collagen (Feige  et al., 1989  ).	bind
22668	1	7190	6	13	NULL	NULL	NULL	FXI	GP		bind		directly			GPIbalpha fragment	GP		His1 - Glu282		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_47_49323_s_179	15375170	2) FXI binds directly to the GPIbalpha fragment His1 - Glu282 and to glycocalicin with almost identical affinity ( Kd of  10 nM) in the presence of ZnCl2 ( Fig. 2).	bind
22669	2	7190	6	13	NULL	NULL	NULL	FXI	GP		bind		directly			glycocalicin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_47_49323_s_179	15375170	2) FXI binds directly to the GPIbalpha fragment His1 - Glu282 and to glycocalicin with almost identical affinity ( Kd of  10 nM) in the presence of ZnCl2 ( Fig. 2).	bind
22670	3	7190	6	13	NULL	NULL	NULL	statement 1	Process		has equal affinity as					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_47_49323_s_179	15375170	2) FXI binds directly to the GPIbalpha fragment His1 - Glu282 and to glycocalicin with almost identical affinity ( Kd of  10 nM) in the presence of ZnCl2 ( Fig. 2).	bind
22671	4	7190	6	13	NULL	NULL	NULL	statement 1	Process		occurs in presence of					ZnCl2	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_47_49323_s_179	15375170	2) FXI binds directly to the GPIbalpha fragment His1 - Glu282 and to glycocalicin with almost identical affinity ( Kd of  10 nM) in the presence of ZnCl2 ( Fig. 2).	bind
22672	5	7190	6	13	NULL	NULL	NULL	statement 2	Process		occurs in presence of					ZnCl2	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_47_49323_s_179	15375170	2) FXI binds directly to the GPIbalpha fragment His1 - Glu282 and to glycocalicin with almost identical affinity ( Kd of  10 nM) in the presence of ZnCl2 ( Fig. 2).	bind
27008	1	7190	7	NULL	NULL	0	NULL	FXI 	NULL		binds	NULL	directly			GPIbalpha fragment	NULL		His1 - Glu282		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_47_49323_s_179	15375170	2) FXI binds directly to the GPIbalpha fragment His1 - Glu282 and to glycocalicin with almost identical affinity ( Kd of  10 nM) in the presence of ZnCl2 ( Fig. 2).	bind
27009	2	7190	7	NULL	NULL	0	NULL	FXI	NULL		binds	NULL	directly			glycocalicin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_47_49323_s_179	15375170	2) FXI binds directly to the GPIbalpha fragment His1 - Glu282 and to glycocalicin with almost identical affinity ( Kd of  10 nM) in the presence of ZnCl2 ( Fig. 2).	bind
27010	3	7190	7	NULL	NULL	0	NULL	statement 1	NULL	affinity of	is identical to	NULL				statement 2	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_47_49323_s_179	15375170	2) FXI binds directly to the GPIbalpha fragment His1 - Glu282 and to glycocalicin with almost identical affinity ( Kd of  10 nM) in the presence of ZnCl2 ( Fig. 2).	bind
27011	4	7190	7	NULL	NULL	0	NULL	statement 1	NULL		in presence of	NULL				ZnCl2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_47_49323_s_179	15375170	2) FXI binds directly to the GPIbalpha fragment His1 - Glu282 and to glycocalicin with almost identical affinity ( Kd of  10 nM) in the presence of ZnCl2 ( Fig. 2).	bind
27012	5	7190	7	NULL	NULL	0	NULL	statement 2	NULL		in presence of	NULL				ZnCl2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_47_49323_s_179	15375170	2) FXI binds directly to the GPIbalpha fragment His1 - Glu282 and to glycocalicin with almost identical affinity ( Kd of  10 nM) in the presence of ZnCl2 ( Fig. 2).	bind
22673	1	7191	6	13	NULL	NULL	NULL	mAb 60.11	GP		bind					gC1qR	GP		NH2-terminal site residues 76 - 93		NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_106_10_1239_s_211	11086025	2) have been used for this study: mAb 60.11 binds to an NH2-terminal site spanning amino acid residues 76 - 93 of gC1qR, and mAb 74.5.	bind
22674	2	7191	6	13	NULL	NULL	NULL	mAb 60.11	GP		bind					mAb 74.5	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_106_10_1239_s_211	11086025	2) have been used for this study: mAb 60.11 binds to an NH2-terminal site spanning amino acid residues 76 - 93 of gC1qR, and mAb 74.5.	bind
27579	1	7191	7	NULL	NULL	0	NULL	 mAb 60.11	NULL		binds to	NULL				gC1qR	NULL		NH2-terminal site residues 76 - 93		NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_106_10_1239_s_211	11086025	2) have been used for this study: mAb 60.11 binds to an NH2-terminal site spanning amino acid residues 76 - 93 of gC1qR, and mAb 74.5.	bind
27581	2	7191	7	NULL	NULL	0	NULL	mAb 60.11 	NULL		binds to	NULL				mAb 74.5	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_106_10_1239_s_211	11086025	2) have been used for this study: mAb 60.11 binds to an NH2-terminal site spanning amino acid residues 76 - 93 of gC1qR, and mAb 74.5.	bind
22675	1	7192	6	13	NULL	NULL	NULL	heparin	Chemical		bind					flXa	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_32_23066_s_227	16766524	2) Heparin binding to fIXa in part counteracts the steric protection provided by Lys98.	bind
22676	2	7192	6	13	NULL	NULL	NULL	statement 1	Process		counteracts 							steric protection provided by	Lys98		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_32_23066_s_227	16766524	2) Heparin binding to fIXa in part counteracts the steric protection provided by Lys98.	bind
27587	1	7192	7	NULL	NULL	0	NULL	Heparin 	NULL		binds to	NULL				fIXa	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23066_s_227	16766524	2) Heparin binding to fIXa in part counteracts the steric protection provided by Lys98.	bind
27588	2	7192	7	NULL	NULL	0	NULL	statement 1	NULL		counteracts	NULL					NULL	steric protection by	Lys98		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_32_23066_s_227	16766524	2) Heparin binding to fIXa in part counteracts the steric protection provided by Lys98.	bind
22677	1	7193	6	13	NULL	NULL	NULL	SP-B21 T cells	Cell	hIL-4-responsive;;human	bind					hIL-4	GP		Y124D		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_23_13869_s_90	7775445	2) hIL-4-responsive human SP-B21  T cells bind hIL-4.Y124D at this same affinity, but bind hIL-4   100-fold more avidly.	bind
22678	2	7193	6	13	NULL	NULL	NULL	SP-B21 T cells	Cell	hIL-4-responsive;;human	bind					hIL-4	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_23_13869_s_90	7775445	2) hIL-4-responsive human SP-B21  T cells bind hIL-4.Y124D at this same affinity, but bind hIL-4   100-fold more avidly.	bind
22921	3	7193	6	13	NULL	NULL	NULL	statement 2	Process		is more avid than					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_23_13869_s_90	7775445	2) hIL-4-responsive human SP-B21  T cells bind hIL-4.Y124D at this same affinity, but bind hIL-4   100-fold more avidly.	bind
27591	1	7193	7	10	NULL	0	NULL	 SP-B21 T cells	NULL	hIL-4-responsive;;human	bind	NULL				hIL-4	NULL		Y124D		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_23_13869_s_90	7775445	2) hIL-4-responsive human SP-B21  T cells bind hIL-4.Y124D at this same affinity, but bind hIL-4   100-fold more avidly.	bind
27592	2	7193	7	10	NULL	0	NULL	SP-B21 T cells	NULL	hIL-4-responsive;;human	bind	NULL	avidly			hIL-4	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_23_13869_s_90	7775445	2) hIL-4-responsive human SP-B21  T cells bind hIL-4.Y124D at this same affinity, but bind hIL-4   100-fold more avidly.	bind
27593	3	7193	7	10	NULL	0	NULL	statement 2	NULL		is more avid than	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_23_13869_s_90	7775445	2) hIL-4-responsive human SP-B21  T cells bind hIL-4.Y124D at this same affinity, but bind hIL-4   100-fold more avidly.	bind
22679	1	7194	6	13	NULL	NULL	NULL	GTPgammaS	Chemical		bind					Gq/11	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_59_4_886_s_36	11259634	2) M1 muscarinic receptors facilitate [35]GTPgammaS binding to Gq/11 and Gi/o proteins (Lazareno and Birdsall 1993  ; DeLapp et al., 1999  ).	bind
22680	2	7194	6	13	NULL	NULL	NULL	GTPgammaS	Chemical		bind					Gi/o proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_59_4_886_s_36	11259634	2) M1 muscarinic receptors facilitate [35]GTPgammaS binding to Gq/11 and Gi/o proteins (Lazareno and Birdsall 1993  ; DeLapp et al., 1999  ).	bind
22681	3	7194	6	13	NULL	NULL	NULL	M1 muscarinic receptors	GP		facilitate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_59_4_886_s_36	11259634	2) M1 muscarinic receptors facilitate [35]GTPgammaS binding to Gq/11 and Gi/o proteins (Lazareno and Birdsall 1993  ; DeLapp et al., 1999  ).	bind
22682	4	7194	6	13	NULL	NULL	NULL	M1 muscarinic receptors	GP		facilitate					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_59_4_886_s_36	11259634	2) M1 muscarinic receptors facilitate [35]GTPgammaS binding to Gq/11 and Gi/o proteins (Lazareno and Birdsall 1993  ; DeLapp et al., 1999  ).	bind
27594	1	7194	7	10	NULL	0	NULL	GTPgammaS	NULL		bind	NULL				Gq/11 protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_59_4_886_s_36	11259634	2) M1 muscarinic receptors facilitate [35]GTPgammaS binding to Gq/11 and Gi/o proteins (Lazareno and Birdsall 1993  ; DeLapp et al., 1999  ).	bind
27595	2	7194	7	10	NULL	0	NULL	GTPgammaS	NULL		bind	NULL				Gi/o protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_59_4_886_s_36	11259634	2) M1 muscarinic receptors facilitate [35]GTPgammaS binding to Gq/11 and Gi/o proteins (Lazareno and Birdsall 1993  ; DeLapp et al., 1999  ).	bind
27596	3	7194	7	NULL	NULL	0	NULL	M1 muscarinic receptors	NULL		facilitate	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_59_4_886_s_36	11259634	2) M1 muscarinic receptors facilitate [35]GTPgammaS binding to Gq/11 and Gi/o proteins (Lazareno and Birdsall 1993  ; DeLapp et al., 1999  ).	bind
27597	4	7194	7	NULL	NULL	0	NULL	M1 muscarinic receptors	NULL		facilitate	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_59_4_886_s_36	11259634	2) M1 muscarinic receptors facilitate [35]GTPgammaS binding to Gq/11 and Gi/o proteins (Lazareno and Birdsall 1993  ; DeLapp et al., 1999  ).	bind
22683	1	7195	6	13	NULL	NULL	NULL	TM1	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_14_14039_s_309	14722123	2) Modification of the N terminus decreases TM1 binding to actin which allows cofilin-mediated cytoskeletal disorganization.	bind
22684	2	7195	6	13	NULL	NULL	NULL			modification of	decreases			N terminus		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_14_14039_s_309	14722123	2) Modification of the N terminus decreases TM1 binding to actin which allows cofilin-mediated cytoskeletal disorganization.	bind
22685	3	7195	6	13	NULL	NULL	NULL	cofilin	GP		mediates					cytoskeletal disorganization	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_14_14039_s_309	14722123	2) Modification of the N terminus decreases TM1 binding to actin which allows cofilin-mediated cytoskeletal disorganization.	bind
22686	4	7195	6	13	NULL	NULL	NULL	statement 1	Process		allows					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_14_14039_s_309	14722123	2) Modification of the N terminus decreases TM1 binding to actin which allows cofilin-mediated cytoskeletal disorganization.	bind
27598	1	7195	7	NULL	NULL	0	NULL	TM1 	NULL		binds to	NULL				actin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_14_14039_s_309	14722123	2) Modification of the N terminus decreases TM1 binding to actin which allows cofilin-mediated cytoskeletal disorganization.	bind
27599	2	7195	7	NULL	NULL	0	NULL		NULL	modification of	decreases	NULL		N terminus		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_14_14039_s_309	14722123	2) Modification of the N terminus decreases TM1 binding to actin which allows cofilin-mediated cytoskeletal disorganization.	bind
27600	3	7195	7	NULL	NULL	0	NULL	cofilin	NULL		mediates	NULL				cytoskeletal disorganization	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_14_14039_s_309	14722123	2) Modification of the N terminus decreases TM1 binding to actin which allows cofilin-mediated cytoskeletal disorganization.	bind
27601	4	7195	7	NULL	NULL	0	NULL	statement 2	NULL		allows	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_14_14039_s_309	14722123	2) Modification of the N terminus decreases TM1 binding to actin which allows cofilin-mediated cytoskeletal disorganization.	bind
22926	1	7196	6	13	NULL	NULL	NULL	mannitol	Chemical		bind								C domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_16_12756_s_24	11278734	2) Modification or mutagenesis of the phosphorylation site in the B domain as well as removal of the cytoplasmic domains changes the mannitol binding kinetics of the C domain ( 11,  12).	bind
22927	2	7196	6	13	NULL	NULL	NULL			mutagenesis of	changes			phosphorylation site in the B domain		statement 1	Process	kinetics of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_16_12756_s_24	11278734	2) Modification or mutagenesis of the phosphorylation site in the B domain as well as removal of the cytoplasmic domains changes the mannitol binding kinetics of the C domain ( 11,  12).	bind
22928	3	7196	6	13	NULL	NULL	NULL			removal of	changes			cytoplasmic domain		statement 1	Process	kinetics of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_16_12756_s_24	11278734	2) Modification or mutagenesis of the phosphorylation site in the B domain as well as removal of the cytoplasmic domains changes the mannitol binding kinetics of the C domain ( 11,  12).	bind
27602	1	7196	7	NULL	NULL	0	NULL	mannitol	NULL		binds	NULL					NULL		C domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_16_12756_s_24	11278734	2) Modification or mutagenesis of the phosphorylation site in the B domain as well as removal of the cytoplasmic domains changes the mannitol binding kinetics of the C domain ( 11,  12).	bind
27603	2	7196	7	NULL	NULL	0	NULL		NULL	mutation of	changes	NULL		 B domain phosphorylation site		statement 1	NULL	binding kinetics of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_16_12756_s_24	11278734	2) Modification or mutagenesis of the phosphorylation site in the B domain as well as removal of the cytoplasmic domains changes the mannitol binding kinetics of the C domain ( 11,  12).	bind
27604	3	7196	7	NULL	NULL	0	NULL		NULL	removal of	changes	NULL		cytoplasmic domain		statement 1	NULL	binding kinetics of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_16_12756_s_24	11278734	2) Modification or mutagenesis of the phosphorylation site in the B domain as well as removal of the cytoplasmic domains changes the mannitol binding kinetics of the C domain ( 11,  12).	bind
22687	1	7197	6	13	NULL	NULL	NULL	fibrinogen	GP		bind					Rap1b	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25715_s_181	11994301	2) Modulation of fibrinogen binding by Rap1b appears to be due primarily to effects on alphaIIbbeta3 affinity.	bind
22688	2	7197	6	13	NULL	NULL	NULL	alphaIIbbeta3	GP	affinity of	effects					statement 1	Process	 modulation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25715_s_181	11994301	2) Modulation of fibrinogen binding by Rap1b appears to be due primarily to effects on alphaIIbbeta3 affinity.	bind
27605	1	7197	7	NULL	NULL	0	NULL	Rap1b	NULL		bind	NULL				fibrinogen	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_28_25715_s_181	11994301	2) Modulation of fibrinogen binding by Rap1b appears to be due primarily to effects on alphaIIbbeta3 affinity.	bind
27606	2	7197	7	NULL	NULL	0	NULL	alphaIIbbeta3	NULL	affinity of	effects	NULL				statement 1	NULL	modulation  of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25715_s_181	11994301	2) Modulation of fibrinogen binding by Rap1b appears to be due primarily to effects on alphaIIbbeta3 affinity.	bind
22689	1	7198	6	13	NULL	NULL	NULL	Monoclonal antibodies	GP		are specific for					Stat1	GP		SH2 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27954_s_244	8910398	2) Monoclonal antibodies specific for the Stat1 SH2 domain block binding of purified latent Stat1 to the tyrosine-phosphorylated IFNgamma receptor docking site ( 24,  25).	bind
22690	2	7198	6	13	NULL	NULL	NULL	Stat1	GP	purified latent	bind					IFNgamma receptor 	GP		tyrosine-phosphorylated docking site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27954_s_244	8910398	2) Monoclonal antibodies specific for the Stat1 SH2 domain block binding of purified latent Stat1 to the tyrosine-phosphorylated IFNgamma receptor docking site ( 24,  25).	bind
22691	3	7198	6	13	NULL	NULL	NULL	statement 1	Process		block					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27954_s_244	8910398	2) Monoclonal antibodies specific for the Stat1 SH2 domain block binding of purified latent Stat1 to the tyrosine-phosphorylated IFNgamma receptor docking site ( 24,  25).	bind
27607	1	7198	7	NULL	NULL	0	NULL	Stat1	NULL	purified latent	bind	NULL				 IFNgamma receptor	NULL		tyrosine-phosphorylated docking site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27954_s_244	8910398	2) Monoclonal antibodies specific for the Stat1 SH2 domain block binding of purified latent Stat1 to the tyrosine-phosphorylated IFNgamma receptor docking site ( 24,  25).	bind
27608	3	7198	7	NULL	NULL	0	NULL	statement 2	NULL		block	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27954_s_244	8910398	2) Monoclonal antibodies specific for the Stat1 SH2 domain block binding of purified latent Stat1 to the tyrosine-phosphorylated IFNgamma receptor docking site ( 24,  25).	bind
37634	2	7198	7	NULL	NULL	0	NULL	Monoclonal antibodies	NULL		are specific for	NULL				Stat1	NULL		SH2 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27954_s_244	8910398	2) Monoclonal antibodies specific for the Stat1 SH2 domain block binding of purified latent Stat1 to the tyrosine-phosphorylated IFNgamma receptor docking site ( 24,  25).	bind
22692	1	7199	6	13	NULL	NULL	NULL	GRK1	GP		bind								PDEdelta		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_1_407_s_236	14561760	2) Mutations in the C AAX box motif-disabling prenylation eliminate the binding of GRK1 to PDEdelta, suggesting that for some interacting partners the lipid attachment is essential.	bind
22693	2	7199	6	13	NULL	NULL	NULL			mutant	disable				C AAX box motif	prenylation	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_1_407_s_236	14561760	2) Mutations in the C AAX box motif-disabling prenylation eliminate the binding of GRK1 to PDEdelta, suggesting that for some interacting partners the lipid attachment is essential.	bind
22694	3	7199	6	13	NULL	NULL	NULL	statement 2	Process		eliminate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_1_407_s_236	14561760	2) Mutations in the C AAX box motif-disabling prenylation eliminate the binding of GRK1 to PDEdelta, suggesting that for some interacting partners the lipid attachment is essential.	bind
27609	1	7199	7	NULL	NULL	0	NULL	GRK1	NULL		bind	NULL					NULL		PDEdelta		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_1_407_s_236	14561760	2) Mutations in the C AAX box motif-disabling prenylation eliminate the binding of GRK1 to PDEdelta, suggesting that for some interacting partners the lipid attachment is essential.	bind
27610	2	7199	7	10	NULL	0	NULL		NULL	mutant	disables	NULL			C AAX box motif	prenylation	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_1_407_s_236	14561760	2) Mutations in the C AAX box motif-disabling prenylation eliminate the binding of GRK1 to PDEdelta, suggesting that for some interacting partners the lipid attachment is essential.	bind
27611	3	7199	7	10	NULL	0	NULL	statement 2	NULL		eliminate	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_1_407_s_236	14561760	2) Mutations in the C AAX box motif-disabling prenylation eliminate the binding of GRK1 to PDEdelta, suggesting that for some interacting partners the lipid attachment is essential.	bind
22695	1	7200	6	13	NULL	NULL	NULL	N1	GP		bind					ANS	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_13_7448_s_74	9516443	2) Only N1 binds with ANS and ATP.	bind
22696	2	7200	6	13	NULL	NULL	NULL	N1	GP		bind					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_13_7448_s_74	9516443	2) Only N1 binds with ANS and ATP.	bind
27612	1	7200	7	NULL	NULL	0	NULL	N1	NULL		binds	NULL				ANS	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_13_7448_s_74	9516443	2) Only N1 binds with ANS and ATP.	bind
27613	2	7200	7	NULL	NULL	0	NULL	N1	NULL		binds	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_13_7448_s_74	9516443	2) Only N1 binds with ANS and ATP.	bind
22697	2	7201	6	13	NULL	NULL	NULL	p47 phox	GP		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_311	11733522	2) p47 phox binds not only to the proline-rich region located at residues 151-160 in the C-terminal cytosolic part of p22 phox but also to a domain, consisting of residues 51-63, located on a loop exposed to the cytosol.	bind
22698	3	7201	6	13	NULL	NULL	NULL	p47 phox	GP		bind					p22 phox	GP		residues 51-63		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_311	11733522	2) p47 phox binds not only to the proline-rich region located at residues 151-160 in the C-terminal cytosolic part of p22 phox but also to a domain, consisting of residues 51-63, located on a loop exposed to the cytosol.	bind
46490	1	7201	6	13	NULL	NULL	NULL	p22 phox	GP		is located in			proline-rich region		p22 phox	GP		residues 151-160 in C-terminal cytosolic part		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_311	11733522	2) p47 phox binds not only to the proline-rich region located at residues 151-160 in the C-terminal cytosolic part of p22 phox but also to a domain, consisting of residues 51-63, located on a loop exposed to the cytosol.	bind
46491	4	7201	6	13	NULL	NULL	NULL	loop	GP		is exposed to					cytosol	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_311	11733522	2) p47 phox binds not only to the proline-rich region located at residues 151-160 in the C-terminal cytosolic part of p22 phox but also to a domain, consisting of residues 51-63, located on a loop exposed to the cytosol.	bind
46492	5	7201	6	13	NULL	NULL	NULL	p22 phox	GP		is located on			residues 51-63		statement 4	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_311	11733522	2) p47 phox binds not only to the proline-rich region located at residues 151-160 in the C-terminal cytosolic part of p22 phox but also to a domain, consisting of residues 51-63, located on a loop exposed to the cytosol.	bind
27614	2	7201	7	10	NULL	0	NULL	p47 phox	NULL		bind	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_311	11733522	2) p47 phox binds not only to the proline-rich region located at residues 151-160 in the C-terminal cytosolic part of p22 phox but also to a domain, consisting of residues 51-63, located on a loop exposed to the cytosol.	bind
27615	3	7201	7	10	NULL	0	NULL	p47 phox	NULL		bind	NULL				p22 phox 	NULL		residues 51-63		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_311	11733522	2) p47 phox binds not only to the proline-rich region located at residues 151-160 in the C-terminal cytosolic part of p22 phox but also to a domain, consisting of residues 51-63, located on a loop exposed to the cytosol.	bind
46493	1	7201	7	10	NULL	0	NULL	p22 phox	NULL		is located in	NULL		proline-rich region		p22 phox	NULL		residues 151-160 in C-terminal cytosolic part		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_311	11733522	2) p47 phox binds not only to the proline-rich region located at residues 151-160 in the C-terminal cytosolic part of p22 phox but also to a domain, consisting of residues 51-63, located on a loop exposed to the cytosol.	bind
46494	4	7201	7	10	NULL	0	NULL	loop	NULL		is exposed to	NULL				cytosol	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_311	11733522	2) p47 phox binds not only to the proline-rich region located at residues 151-160 in the C-terminal cytosolic part of p22 phox but also to a domain, consisting of residues 51-63, located on a loop exposed to the cytosol.	bind
46495	5	7201	7	10	NULL	0	NULL	p22 phox	NULL		is located on	NULL		residues 51-63		statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_311	11733522	2) p47 phox binds not only to the proline-rich region located at residues 151-160 in the C-terminal cytosolic part of p22 phox but also to a domain, consisting of residues 51-63, located on a loop exposed to the cytosol.	bind
22699	1	7204	6	13	NULL	NULL	NULL	TFPI	GP		bind					hepatoma cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_42_25873_s_29	8824219	2) Protamine, which competes for HSPG-binding sites, inhibits TFPI binding to hepatoma cells and prolongs the half-life of 125I-TFPI in mice ( 19).	bind
22700	2	7204	6	13	NULL	NULL	NULL	Protamine	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_42_25873_s_29	8824219	2) Protamine, which competes for HSPG-binding sites, inhibits TFPI binding to hepatoma cells and prolongs the half-life of 125I-TFPI in mice ( 19).	bind
22701	3	7204	6	13	NULL	NULL	NULL	Protamine	GP		competes for								HSPG binding sites		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_42_25873_s_29	8824219	2) Protamine, which competes for HSPG-binding sites, inhibits TFPI binding to hepatoma cells and prolongs the half-life of 125I-TFPI in mice ( 19).	bind
53363	4	7204	6	13	NULL	NULL	NULL	Protamine	GP		prolonges					125I-TFPI	GP	half-life of;;mice			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_42_25873_s_29	8824219	2) Protamine, which competes for HSPG-binding sites, inhibits TFPI binding to hepatoma cells and prolongs the half-life of 125I-TFPI in mice ( 19).	bind
27616	1	7204	7	NULL	NULL	0	NULL	TFPI	NULL		bind	NULL				hepatoma cells	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_42_25873_s_29	8824219	2) Protamine, which competes for HSPG-binding sites, inhibits TFPI binding to hepatoma cells and prolongs the half-life of 125I-TFPI in mice ( 19).	bind
27617	2	7204	7	NULL	NULL	0	NULL	Protamine	NULL		competes for	NULL					NULL		HSPG-binding sites		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_42_25873_s_29	8824219	2) Protamine, which competes for HSPG-binding sites, inhibits TFPI binding to hepatoma cells and prolongs the half-life of 125I-TFPI in mice ( 19).	bind
27618	3	7204	7	NULL	NULL	0	NULL	Protamine	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_42_25873_s_29	8824219	2) Protamine, which competes for HSPG-binding sites, inhibits TFPI binding to hepatoma cells and prolongs the half-life of 125I-TFPI in mice ( 19).	bind
27619	4	7204	7	10	NULL	0	NULL	Protamine	NULL		prolongs	NULL				125I-TFPI	NULL	half-life of;;mice			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_42_25873_s_29	8824219	2) Protamine, which competes for HSPG-binding sites, inhibits TFPI binding to hepatoma cells and prolongs the half-life of 125I-TFPI in mice ( 19).	bind
22702	1	7205	6	13	NULL	NULL	NULL	PAFAH-45	GP		bind			WD40 repeats		beta-adrenergic receptor kinase	GP		PH domain		NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_biochem-biophys-res-commun_209_2_7733932_s_5	7733932	2) Protein constructs expressing all 7 WD40 repeats of PAFAH-45  but lacking the N-terminal non WD40 region also bind PH domains of beta-adrenergic  receptor kinase, beta-spectrin, TecIIa and dynamin but with a differing  hierarchy of affinities than that seen with G beta.	bind
22703	2	7205	6	13	NULL	NULL	NULL	PAFAH-45	GP		bind			WD40 repeats		beta-spectrin	GP		PH domain		NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_biochem-biophys-res-commun_209_2_7733932_s_5	7733932	2) Protein constructs expressing all 7 WD40 repeats of PAFAH-45  but lacking the N-terminal non WD40 region also bind PH domains of beta-adrenergic  receptor kinase, beta-spectrin, TecIIa and dynamin but with a differing  hierarchy of affinities than that seen with G beta.	bind
22704	3	7205	6	13	NULL	NULL	NULL	PAFAH-45	GP		bind			WD40 repeats		TecIIa	GP		PH domain		NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_biochem-biophys-res-commun_209_2_7733932_s_5	7733932	2) Protein constructs expressing all 7 WD40 repeats of PAFAH-45  but lacking the N-terminal non WD40 region also bind PH domains of beta-adrenergic  receptor kinase, beta-spectrin, TecIIa and dynamin but with a differing  hierarchy of affinities than that seen with G beta.	bind
22705	4	7205	6	13	NULL	NULL	NULL	PAFAH-45	GP		bind			WD40 repeats		Dynamin	GP		PH domain		NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_biochem-biophys-res-commun_209_2_7733932_s_5	7733932	2) Protein constructs expressing all 7 WD40 repeats of PAFAH-45  but lacking the N-terminal non WD40 region also bind PH domains of beta-adrenergic  receptor kinase, beta-spectrin, TecIIa and dynamin but with a differing  hierarchy of affinities than that seen with G beta.	bind
23107	5	7205	6	13	NULL	NULL	NULL	PAFAH-45	GP		bind			WD40 repeats		G beta	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_biochem-biophys-res-commun_209_2_7733932_s_5	7733932	2) Protein constructs expressing all 7 WD40 repeats of PAFAH-45  but lacking the N-terminal non WD40 region also bind PH domains of beta-adrenergic  receptor kinase, beta-spectrin, TecIIa and dynamin but with a differing  hierarchy of affinities than that seen with G beta.	bind
53364	6	7205	6	13	NULL	NULL	NULL	PAFAH-45	GP		lacks								N-terminal non WD40 region		NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_biochem-biophys-res-commun_209_2_7733932_s_5	7733932	2) Protein constructs expressing all 7 WD40 repeats of PAFAH-45  but lacking the N-terminal non WD40 region also bind PH domains of beta-adrenergic  receptor kinase, beta-spectrin, TecIIa and dynamin but with a differing  hierarchy of affinities than that seen with G beta.	bind
27620	1	7205	7	NULL	NULL	0	NULL	PAFAH-45	NULL		bind	NULL		WD40 repeat		beta-adrenergic receptor kinase	NULL		PH domain		NULL		0	NULL	NULL	NULL	abs-batch0517-0529_biochem-biophys-res-commun_209_2_7733932_s_5	7733932	2) Protein constructs expressing all 7 WD40 repeats of PAFAH-45  but lacking the N-terminal non WD40 region also bind PH domains of beta-adrenergic  receptor kinase, beta-spectrin, TecIIa and dynamin but with a differing  hierarchy of affinities than that seen with G beta.	bind
27621	2	7205	7	NULL	NULL	0	NULL	PAFAH-45	NULL		bind	NULL		WD40 repeat		beta-spectrin	NULL		PH domain		NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_biochem-biophys-res-commun_209_2_7733932_s_5	7733932	2) Protein constructs expressing all 7 WD40 repeats of PAFAH-45  but lacking the N-terminal non WD40 region also bind PH domains of beta-adrenergic  receptor kinase, beta-spectrin, TecIIa and dynamin but with a differing  hierarchy of affinities than that seen with G beta.	bind
27622	3	7205	7	NULL	NULL	0	NULL	PAFAH-45	NULL		bind	NULL		WD40 repeat		TecIIa	NULL		PH domain		NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_biochem-biophys-res-commun_209_2_7733932_s_5	7733932	2) Protein constructs expressing all 7 WD40 repeats of PAFAH-45  but lacking the N-terminal non WD40 region also bind PH domains of beta-adrenergic  receptor kinase, beta-spectrin, TecIIa and dynamin but with a differing  hierarchy of affinities than that seen with G beta.	bind
27623	4	7205	7	NULL	NULL	0	NULL	PAFAH-45	NULL		bind	NULL		WD40 repeat		dynamin	NULL		PH domain		NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_biochem-biophys-res-commun_209_2_7733932_s_5	7733932	2) Protein constructs expressing all 7 WD40 repeats of PAFAH-45  but lacking the N-terminal non WD40 region also bind PH domains of beta-adrenergic  receptor kinase, beta-spectrin, TecIIa and dynamin but with a differing  hierarchy of affinities than that seen with G beta.	bind
27624	5	7205	7	NULL	NULL	0	NULL	PAFAH-45	NULL		bind	NULL		WD40 repeat		Gbeta	NULL				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_biochem-biophys-res-commun_209_2_7733932_s_5	7733932	2) Protein constructs expressing all 7 WD40 repeats of PAFAH-45  but lacking the N-terminal non WD40 region also bind PH domains of beta-adrenergic  receptor kinase, beta-spectrin, TecIIa and dynamin but with a differing  hierarchy of affinities than that seen with G beta.	bind
27625	6	7205	7	NULL	NULL	0	NULL	PAFAH-45	NULL		lacks	NULL					NULL		N-terminal non WD40 region		NULL		0	NULL	NULL	NULL	abs-batch0517-0529_biochem-biophys-res-commun_209_2_7733932_s_5	7733932	2) Protein constructs expressing all 7 WD40 repeats of PAFAH-45  but lacking the N-terminal non WD40 region also bind PH domains of beta-adrenergic  receptor kinase, beta-spectrin, TecIIa and dynamin but with a differing  hierarchy of affinities than that seen with G beta.	bind
22706	1	7206	6	13	NULL	NULL	NULL	RAP74	GP		bind					RAP30	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_20_11703_s_207	8662660	2) RAP74 could bind RAP30 to block the TFIIB binding site on  RAP30.	bind
22707	2	7206	6	13	NULL	NULL	NULL	statement 1	Process		block					RAP30	GP		TFIIB binding site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_20_11703_s_207	8662660	2) RAP74 could bind RAP30 to block the TFIIB binding site on  RAP30.	bind
27626	1	7206	7	NULL	NULL	0	NULL	RAP74	NULL		bind	NULL				RAP30	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_20_11703_s_207	8662660	2) RAP74 could bind RAP30 to block the TFIIB binding site on  RAP30.	bind
27627	2	7206	7	NULL	NULL	0	NULL	statement 1	NULL		block	NULL				RAP30	NULL		TFIIB binding site		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_20_11703_s_207	8662660	2) RAP74 could bind RAP30 to block the TFIIB binding site on  RAP30.	bind
22708	1	7207	6	13	NULL	NULL	NULL	ATP	Chemical		bind					DnaK	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_11_6137_s_157	8626401	2) The  exogenous P   inhibits both ATP hydrolysis and DnaK  conformational change but does not influence the binding of ATP to DnaK  (this paper).	bind
22709	2	7207	6	13	NULL	NULL	NULL	exogenous P	Chemical		inhibits					ATP	Chemical	hydrolysis of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_11_6137_s_157	8626401	2) The  exogenous P   inhibits both ATP hydrolysis and DnaK  conformational change but does not influence the binding of ATP to DnaK  (this paper).	bind
22710	3	7207	6	13	NULL	NULL	NULL	exogenous P	Chemical		inhibits					DnaK	GP	conformational change of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_11_6137_s_157	8626401	2) The  exogenous P   inhibits both ATP hydrolysis and DnaK  conformational change but does not influence the binding of ATP to DnaK  (this paper).	bind
53365	4	7207	6	13	NULL	NULL	NULL	exogenous P	Chemical		does not influence					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_11_6137_s_157	8626401	2) The  exogenous P   inhibits both ATP hydrolysis and DnaK  conformational change but does not influence the binding of ATP to DnaK  (this paper).	bind
27628	1	7207	7	NULL	NULL	0	NULL	ATP  	NULL		bind	NULL				DnaK	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_11_6137_s_157	8626401	2) The  exogenous P   inhibits both ATP hydrolysis and DnaK  conformational change but does not influence the binding of ATP to DnaK  (this paper).	bind
27629	2	7207	7	NULL	NULL	0	NULL	exogenous P	NULL		inhibits	NULL				ATP	NULL	hydrolysis of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_11_6137_s_157	8626401	2) The  exogenous P   inhibits both ATP hydrolysis and DnaK  conformational change but does not influence the binding of ATP to DnaK  (this paper).	bind
27630	3	7207	7	NULL	NULL	0	NULL	exogenous P	NULL		inhibits	NULL				DnaK	NULL	conformational change of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_11_6137_s_157	8626401	2) The  exogenous P   inhibits both ATP hydrolysis and DnaK  conformational change but does not influence the binding of ATP to DnaK  (this paper).	bind
27631	4	7207	7	NULL	NULL	0	NULL	exogenous P	NULL		does not influence	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_11_6137_s_157	8626401	2) The  exogenous P   inhibits both ATP hydrolysis and DnaK  conformational change but does not influence the binding of ATP to DnaK  (this paper).	bind
22711	1	7208	6	13	NULL	NULL	NULL	Stat3	GP		bind					pY XXQ-containing peptides	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_18967_s_27	14966128	2) The +3 Gln is required for binding of Stat3 to pY XXQ-containing peptides.	bind
22712	2	7208	6	13	NULL	NULL	NULL	Gln	AminoAcid		is required for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_18967_s_27	14966128	2) The +3 Gln is required for binding of Stat3 to pY XXQ-containing peptides.	bind
27632	1	7208	7	10	NULL	0	NULL	 Stat3	NULL		bind	NULL				pY XXQ-containing peptides	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_18967_s_27	14966128	2) The +3 Gln is required for binding of Stat3 to pY XXQ-containing peptides.	bind
27633	2	7208	7	NULL	NULL	0	NULL	Gln	NULL		is required for	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_18_18967_s_27	14966128	2) The +3 Gln is required for binding of Stat3 to pY XXQ-containing peptides.	bind
22717	1	7209	6	13	NULL	NULL	NULL	TSG101/Vps23p	GP		bind			C-terminal region		VPS28/Vps28p	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_34_36059_s_33	15218037	2) The C-terminal region of TSG101/Vps23p binds VPS28/Vps28p ( ,  ,  ).	bind
27634	1	7209	7	NULL	NULL	0	NULL	TSG101/Vps23p	NULL		binds	NULL		C-terminal region		 VPS28/Vps28p	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_34_36059_s_33	15218037	2) The C-terminal region of TSG101/Vps23p binds VPS28/Vps28p ( ,  ,  ).	bind
22719	1	7210	6	13	NULL	NULL	NULL	Cu(I)	Chemical	binding of	signals					APP	GP	processing of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_19_17401_s_172	12611883	2) The Cu(I) binding signals APP processing or proteolytic breakdown via the non-amyloidogenic route ( 21,  22).	bind
22721	2	7210	6	13	NULL	NULL	NULL	Cu(I)	Chemical	binding of	signals					APP	GP	proteolytic breakdown of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_19_17401_s_172	12611883	2) The Cu(I) binding signals APP processing or proteolytic breakdown via the non-amyloidogenic route ( 21,  22).	bind
22724	3	7210	6	13	NULL	NULL	NULL	statement 2	Process		occurs by					non-amyloidogenic route	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_19_17401_s_172	12611883	2) The Cu(I) binding signals APP processing or proteolytic breakdown via the non-amyloidogenic route ( 21,  22).	bind
27635	1	7210	7	NULL	NULL	0	NULL	Cu(I)	NULL	binding of	signals	NULL				APP	NULL	processing of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_19_17401_s_172	12611883	2) The Cu(I) binding signals APP processing or proteolytic breakdown via the non-amyloidogenic route ( 21,  22).	bind
27636	2	7210	7	10	NULL	0	NULL	Cu(I)	NULL	binding of	signals	NULL				APP	NULL	proteolytic breakdown of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_19_17401_s_172	12611883	2) The Cu(I) binding signals APP processing or proteolytic breakdown via the non-amyloidogenic route ( 21,  22).	bind
46496	3	7210	7	10	NULL	0	NULL	statement 2	NULL		via	NULL				non-amyloidogenic route	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_19_17401_s_172	12611883	2) The Cu(I) binding signals APP processing or proteolytic breakdown via the non-amyloidogenic route ( 21,  22).	bind
22727	1	7211	6	13	NULL	NULL	NULL	GAT	GP		is					GGA and Tom1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_8_7105_s_17	14660606	2) The GAT ( GGA  and  Tom1) domain interacts with a GTP-bound form of the small GTPase ADP-ribosylation factor (ARF) and is responsible for association of GGAs with TGN membranes ( - ).	bind
22728	2	7211	6	13	NULL	NULL	NULL	GTP	Chemical		bind					ARF	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_8_7105_s_17	14660606	2) The GAT ( GGA  and  Tom1) domain interacts with a GTP-bound form of the small GTPase ADP-ribosylation factor (ARF) and is responsible for association of GGAs with TGN membranes ( - ).	bind
22729	3	7211	6	13	NULL	NULL	NULL	ARF	GP		is					ADP-ribosylation factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_8_7105_s_17	14660606	2) The GAT ( GGA  and  Tom1) domain interacts with a GTP-bound form of the small GTPase ADP-ribosylation factor (ARF) and is responsible for association of GGAs with TGN membranes ( - ).	bind
22730	4	7211	6	13	NULL	NULL	NULL				interacts with			GAT domain		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_8_7105_s_17	14660606	2) The GAT ( GGA  and  Tom1) domain interacts with a GTP-bound form of the small GTPase ADP-ribosylation factor (ARF) and is responsible for association of GGAs with TGN membranes ( - ).	bind
22731	5	7211	6	13	NULL	NULL	NULL	GGAs	GP		associate with					TGN membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_8_7105_s_17	14660606	2) The GAT ( GGA  and  Tom1) domain interacts with a GTP-bound form of the small GTPase ADP-ribosylation factor (ARF) and is responsible for association of GGAs with TGN membranes ( - ).	bind
22734	6	7211	6	13	NULL	NULL	NULL				is responsible for			GAT domain		statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_8_7105_s_17	14660606	2) The GAT ( GGA  and  Tom1) domain interacts with a GTP-bound form of the small GTPase ADP-ribosylation factor (ARF) and is responsible for association of GGAs with TGN membranes ( - ).	bind
46499	7	7211	6	13	NULL	NULL	NULL	ARF	GP		is a type of					small GTPases	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_8_7105_s_17	14660606	2) The GAT ( GGA  and  Tom1) domain interacts with a GTP-bound form of the small GTPase ADP-ribosylation factor (ARF) and is responsible for association of GGAs with TGN membranes ( - ).	bind
27637	1	7211	7	13	NULL	NULL	NULL				interacts with			GAT domain		statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_8_7105_s_17	14660606	2) The GAT ( GGA  and  Tom1) domain interacts with a GTP-bound form of the small GTPase ADP-ribosylation factor (ARF) and is responsible for association of GGAs with TGN membranes ( - ).	bind
27638	2	7211	7	NULL	NULL	0	NULL		NULL		consist of	NULL		GAT domain			NULL		GGA and Tom1 domain		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_7105_s_17	14660606	2) The GAT ( GGA  and  Tom1) domain interacts with a GTP-bound form of the small GTPase ADP-ribosylation factor (ARF) and is responsible for association of GGAs with TGN membranes ( - ).	bind
27639	3	7211	7	NULL	NULL	0	NULL		NULL		associate with	NULL		GGA		TGN membranes	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_7105_s_17	14660606	2) The GAT ( GGA  and  Tom1) domain interacts with a GTP-bound form of the small GTPase ADP-ribosylation factor (ARF) and is responsible for association of GGAs with TGN membranes ( - ).	bind
27640	4	7211	7	NULL	NULL	0	NULL		NULL		is responsible for	NULL		GAT domain		statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_7105_s_17	14660606	2) The GAT ( GGA  and  Tom1) domain interacts with a GTP-bound form of the small GTPase ADP-ribosylation factor (ARF) and is responsible for association of GGAs with TGN membranes ( - ).	bind
27641	5	7211	7	NULL	NULL	0	NULL	ARF	NULL		is	NULL				ADP-ribosylation factor	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_7105_s_17	14660606	2) The GAT ( GGA  and  Tom1) domain interacts with a GTP-bound form of the small GTPase ADP-ribosylation factor (ARF) and is responsible for association of GGAs with TGN membranes ( - ).	bind
46497	6	7211	7	10	NULL	0	NULL	GTP	NULL		bind	NULL				ARF	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_7105_s_17	14660606	2) The GAT ( GGA  and  Tom1) domain interacts with a GTP-bound form of the small GTPase ADP-ribosylation factor (ARF) and is responsible for association of GGAs with TGN membranes ( - ).	bind
46498	7	7211	7	10	NULL	0	NULL	ARF	NULL		is a type of	NULL				small GTPase	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_7105_s_17	14660606	2) The GAT ( GGA  and  Tom1) domain interacts with a GTP-bound form of the small GTPase ADP-ribosylation factor (ARF) and is responsible for association of GGAs with TGN membranes ( - ).	bind
22741	1	7212	6	13	NULL	NULL	NULL	hnRNP M4	GP	rat	expressed in					E.coli	Organism				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_33_31067_s_266	11406629	2) The rat hnRNP M4 fusion protein expressed in  E. coli binds CEA and this interaction is a Ca2+-dependent process (Fig.  5).	bind
22742	2	7212	6	13	NULL	NULL	NULL	statement 1	GP		bind					CEA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_33_31067_s_266	11406629	2) The rat hnRNP M4 fusion protein expressed in  E. coli binds CEA and this interaction is a Ca2+-dependent process (Fig.  5).	bind
22744	3	7212	6	13	NULL	NULL	NULL	statement 2	Process		is dependent on					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_33_31067_s_266	11406629	2) The rat hnRNP M4 fusion protein expressed in  E. coli binds CEA and this interaction is a Ca2+-dependent process (Fig.  5).	bind
46500	3	7212	6	13	NULL	NULL	NULL	hnRNP M4	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_33_31067_s_266	11406629	2) The rat hnRNP M4 fusion protein expressed in  E. coli binds CEA and this interaction is a Ca2+-dependent process (Fig.  5).	bind
27642	1	7212	7	10	NULL	0	NULL	hnRNP M4	NULL	rat	binds	NULL				CEA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_33_31067_s_266	11406629	2) The rat hnRNP M4 fusion protein expressed in  E. coli binds CEA and this interaction is a Ca2+-dependent process (Fig.  5).	bind
27643	2	7212	7	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				Ca2+	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_33_31067_s_266	11406629	2) The rat hnRNP M4 fusion protein expressed in  E. coli binds CEA and this interaction is a Ca2+-dependent process (Fig.  5).	bind
46501	3	7212	7	10	NULL	0	NULL	hnRNP M4	NULL		is a type of	NULL				fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_33_31067_s_266	11406629	2) The rat hnRNP M4 fusion protein expressed in  E. coli binds CEA and this interaction is a Ca2+-dependent process (Fig.  5).	bind
22748	1	7213	6	13	NULL	NULL	NULL	S4GGnM-R	GP		bind					ligand	GP	soluble	terminal S4GGnM		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_23_14629_s_141	9169424	2) The S4GGnM-R is able to bind soluble ligands terminating with S4GGnM as well as ligands with terminal Man or Fuc in the PEG precipitation assay, whereas the Man-R will bind ligands with terminal Man or Fuc but not those with terminal S4GGnM in the same assay.	bind
22751	2	7213	6	13	NULL	NULL	NULL	S4GGnM-R	GP		bind					ligand	Chemical	soluble	terminal Fuc		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_23_14629_s_141	9169424	2) The S4GGnM-R is able to bind soluble ligands terminating with S4GGnM as well as ligands with terminal Man or Fuc in the PEG precipitation assay, whereas the Man-R will bind ligands with terminal Man or Fuc but not those with terminal S4GGnM in the same assay.	bind
22929	3	7213	6	13	NULL	NULL	NULL	S4GGnM-R	GP		bind					ligand	Chemical	soluble	terminal Man		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_23_14629_s_141	9169424	2) The S4GGnM-R is able to bind soluble ligands terminating with S4GGnM as well as ligands with terminal Man or Fuc in the PEG precipitation assay, whereas the Man-R will bind ligands with terminal Man or Fuc but not those with terminal S4GGnM in the same assay.	bind
22930	4	7213	6	13	NULL	NULL	NULL	ManR	GP		bind					ligand	Chemical	soluble	terminal Man		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_23_14629_s_141	9169424	2) The S4GGnM-R is able to bind soluble ligands terminating with S4GGnM as well as ligands with terminal Man or Fuc in the PEG precipitation assay, whereas the Man-R will bind ligands with terminal Man or Fuc but not those with terminal S4GGnM in the same assay.	bind
22931	5	7213	6	13	NULL	NULL	NULL	ManR	GP		bind					ligand	Chemical	soluble	terminal Fuc		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_23_14629_s_141	9169424	2) The S4GGnM-R is able to bind soluble ligands terminating with S4GGnM as well as ligands with terminal Man or Fuc in the PEG precipitation assay, whereas the Man-R will bind ligands with terminal Man or Fuc but not those with terminal S4GGnM in the same assay.	bind
22932	6	7213	6	13	NULL	NULL	NULL	ManR	GP		does not bind					ligand	Chemical	soluble	terminal S4GGnM		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_23_14629_s_141	9169424	2) The S4GGnM-R is able to bind soluble ligands terminating with S4GGnM as well as ligands with terminal Man or Fuc in the PEG precipitation assay, whereas the Man-R will bind ligands with terminal Man or Fuc but not those with terminal S4GGnM in the same assay.	bind
27644	1	7213	7	10	NULL	0	NULL	S4GGnM-R	NULL		bind	NULL				ligand	NULL	soluble	terminal S4GGnM		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_23_14629_s_141	9169424	2) The S4GGnM-R is able to bind soluble ligands terminating with S4GGnM as well as ligands with terminal Man or Fuc in the PEG precipitation assay, whereas the Man-R will bind ligands with terminal Man or Fuc but not those with terminal S4GGnM in the same assay.	bind
27645	2	7213	7	10	NULL	0	NULL	S4GGnM-R	NULL		bind	NULL				ligand	NULL	soluble	terminal Man		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_23_14629_s_141	9169424	2) The S4GGnM-R is able to bind soluble ligands terminating with S4GGnM as well as ligands with terminal Man or Fuc in the PEG precipitation assay, whereas the Man-R will bind ligands with terminal Man or Fuc but not those with terminal S4GGnM in the same assay.	bind
27646	3	7213	7	10	NULL	0	NULL	S4GGnM-R	NULL		binds	NULL				ligand	NULL	soluble	terminal Fuc		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_23_14629_s_141	9169424	2) The S4GGnM-R is able to bind soluble ligands terminating with S4GGnM as well as ligands with terminal Man or Fuc in the PEG precipitation assay, whereas the Man-R will bind ligands with terminal Man or Fuc but not those with terminal S4GGnM in the same assay.	bind
27647	4	7213	7	10	NULL	0	NULL	 Man-R	NULL		bind	NULL				ligand	NULL	soluble	terminal Man		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_23_14629_s_141	9169424	2) The S4GGnM-R is able to bind soluble ligands terminating with S4GGnM as well as ligands with terminal Man or Fuc in the PEG precipitation assay, whereas the Man-R will bind ligands with terminal Man or Fuc but not those with terminal S4GGnM in the same assay.	bind
27648	5	7213	7	10	NULL	0	NULL	Man-R	NULL		bind	NULL				ligand	NULL	soluble	terminal Fuc		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_23_14629_s_141	9169424	2) The S4GGnM-R is able to bind soluble ligands terminating with S4GGnM as well as ligands with terminal Man or Fuc in the PEG precipitation assay, whereas the Man-R will bind ligands with terminal Man or Fuc but not those with terminal S4GGnM in the same assay.	bind
27649	6	7213	7	10	NULL	0	NULL	Man-R	NULL		does not bind	NULL				ligand	NULL	soluble	terminal S4GGnM		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_23_14629_s_141	9169424	2) The S4GGnM-R is able to bind soluble ligands terminating with S4GGnM as well as ligands with terminal Man or Fuc in the PEG precipitation assay, whereas the Man-R will bind ligands with terminal Man or Fuc but not those with terminal S4GGnM in the same assay.	bind
22755	1	7214	6	13	NULL	NULL	NULL	GST-hTom70	GP	mutant	bind			N267		Mcl-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_9_3952_s_187	16822835	2) The Tom70 mutant containing the N-terminal three TPR domains as in GST-hTom70N267 bound to Mcl-1 with an affinity that was much higher than the mutant without this N-terminal region ( Figure 7B).	bind
22762	2	7214	6	13	NULL	NULL	NULL	GST-hTom70	GP	mutant	bind					Mcl-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_9_3952_s_187	16822835	2) The Tom70 mutant containing the N-terminal three TPR domains as in GST-hTom70N267 bound to Mcl-1 with an affinity that was much higher than the mutant without this N-terminal region ( Figure 7B).	bind
22764	3	7214	6	13	NULL	NULL	NULL	statement 1	Process		higher affinity than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_9_3952_s_187	16822835	2) The Tom70 mutant containing the N-terminal three TPR domains as in GST-hTom70N267 bound to Mcl-1 with an affinity that was much higher than the mutant without this N-terminal region ( Figure 7B).	bind
53366	4	7214	6	13	NULL	NULL	NULL	Tom70	GP	mutant	contains								N-terminal three TPR domains		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_9_3952_s_187	16822835	2) The Tom70 mutant containing the N-terminal three TPR domains as in GST-hTom70N267 bound to Mcl-1 with an affinity that was much higher than the mutant without this N-terminal region ( Figure 7B).	bind
27650	1	7214	7	NULL	NULL	0	NULL	GST-hTom70	NULL	mutant	bind	NULL		N267		Mcl-1	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_9_3952_s_187	16822835	2) The Tom70 mutant containing the N-terminal three TPR domains as in GST-hTom70N267 bound to Mcl-1 with an affinity that was much higher than the mutant without this N-terminal region ( Figure 7B).	bind
27651	2	7214	7	NULL	NULL	0	NULL	Tom70	NULL	mutant	contains	NULL					NULL		N-terminal three TPR domains		NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_9_3952_s_187	16822835	2) The Tom70 mutant containing the N-terminal three TPR domains as in GST-hTom70N267 bound to Mcl-1 with an affinity that was much higher than the mutant without this N-terminal region ( Figure 7B).	bind
27654	3	7214	7	NULL	NULL	0	NULL	Tom70	NULL	mutant lacking	bind	NULL		 N-terminal TPR domain		Mcl-1 	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_9_3952_s_187	16822835	2) The Tom70 mutant containing the N-terminal three TPR domains as in GST-hTom70N267 bound to Mcl-1 with an affinity that was much higher than the mutant without this N-terminal region ( Figure 7B).	bind
27656	4	7214	7	10	NULL	0	NULL	statement 1	NULL		higher affinity than	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_9_3952_s_187	16822835	2) The Tom70 mutant containing the N-terminal three TPR domains as in GST-hTom70N267 bound to Mcl-1 with an affinity that was much higher than the mutant without this N-terminal region ( Figure 7B).	bind
22782	1	7216	6	13	NULL	NULL	NULL				bind			Tyr(P)527					SH2 domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_33_23776_s_280	16790421	2) Tyr(P)527 binds to the SH2 domain.	bind
27661	1	7216	7	NULL	NULL	0	NULL		NULL		binds to	NULL		Tyr(P)527			NULL		SH2 domain		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_33_23776_s_280	16790421	2) Tyr(P)527 binds to the SH2 domain.	bind
22785	1	7217	6	13	NULL	NULL	NULL	VPAC1 receptor	GP		bind					vasoactive intestinal polypeptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_26_23562_s_31	11320087	2) VPAC1 and VPAC2 receptors, which bind both vasoactive intestinal polypeptide and PACAP but activate almost exclusively adenylate cyclase ( 19-21) and have been found in lung, liver, prostate gland, and seminal vesicles.	bind
22786	2	7217	6	13	NULL	NULL	NULL	VPAC1 receptor	GP		bind					PACAP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_26_23562_s_31	11320087	2) VPAC1 and VPAC2 receptors, which bind both vasoactive intestinal polypeptide and PACAP but activate almost exclusively adenylate cyclase ( 19-21) and have been found in lung, liver, prostate gland, and seminal vesicles.	bind
22788	3	7217	6	13	NULL	NULL	NULL	VPAC2 receptor	GP		bind					vasoactive intestinal polypeptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_26_23562_s_31	11320087	2) VPAC1 and VPAC2 receptors, which bind both vasoactive intestinal polypeptide and PACAP but activate almost exclusively adenylate cyclase ( 19-21) and have been found in lung, liver, prostate gland, and seminal vesicles.	bind
22789	4	7217	6	13	NULL	NULL	NULL	VPAC2 receptor	GP		bind					PACAP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_26_23562_s_31	11320087	2) VPAC1 and VPAC2 receptors, which bind both vasoactive intestinal polypeptide and PACAP but activate almost exclusively adenylate cyclase ( 19-21) and have been found in lung, liver, prostate gland, and seminal vesicles.	bind
22790	5	7217	6	13	NULL	NULL	NULL	VPAC1 receptor	GP		activates		exclusively			adenylate cyclase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_26_23562_s_31	11320087	2) VPAC1 and VPAC2 receptors, which bind both vasoactive intestinal polypeptide and PACAP but activate almost exclusively adenylate cyclase ( 19-21) and have been found in lung, liver, prostate gland, and seminal vesicles.	bind
22791	6	7217	6	13	NULL	NULL	NULL	VPAC2 receptor	GP		activate		exclusively			adenylate cyclase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_26_23562_s_31	11320087	2) VPAC1 and VPAC2 receptors, which bind both vasoactive intestinal polypeptide and PACAP but activate almost exclusively adenylate cyclase ( 19-21) and have been found in lung, liver, prostate gland, and seminal vesicles.	bind
22792	7	7217	6	13	NULL	NULL	NULL	VPAC1 receptor	GP		is found in					lung	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_26_23562_s_31	11320087	2) VPAC1 and VPAC2 receptors, which bind both vasoactive intestinal polypeptide and PACAP but activate almost exclusively adenylate cyclase ( 19-21) and have been found in lung, liver, prostate gland, and seminal vesicles.	bind
22793	8	7217	6	13	NULL	NULL	NULL	VPAC1 receptor	GP		is found in					liver	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_26_23562_s_31	11320087	2) VPAC1 and VPAC2 receptors, which bind both vasoactive intestinal polypeptide and PACAP but activate almost exclusively adenylate cyclase ( 19-21) and have been found in lung, liver, prostate gland, and seminal vesicles.	bind
22794	9	7217	6	13	NULL	NULL	NULL	VPAC1 receptor	GP		is found in					prostate gland	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_26_23562_s_31	11320087	2) VPAC1 and VPAC2 receptors, which bind both vasoactive intestinal polypeptide and PACAP but activate almost exclusively adenylate cyclase ( 19-21) and have been found in lung, liver, prostate gland, and seminal vesicles.	bind
22796	10	7217	6	13	NULL	NULL	NULL	VPAC1 receptor	GP		is found in					seminal vesicle	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_26_23562_s_31	11320087	2) VPAC1 and VPAC2 receptors, which bind both vasoactive intestinal polypeptide and PACAP but activate almost exclusively adenylate cyclase ( 19-21) and have been found in lung, liver, prostate gland, and seminal vesicles.	bind
22798	11	7217	6	13	NULL	NULL	NULL	VPAC2 receptor	GP		is found in					lung	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_26_23562_s_31	11320087	2) VPAC1 and VPAC2 receptors, which bind both vasoactive intestinal polypeptide and PACAP but activate almost exclusively adenylate cyclase ( 19-21) and have been found in lung, liver, prostate gland, and seminal vesicles.	bind
22799	12	7217	6	13	NULL	NULL	NULL	VPAC2 receptor	GP		is found in					liver	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_26_23562_s_31	11320087	2) VPAC1 and VPAC2 receptors, which bind both vasoactive intestinal polypeptide and PACAP but activate almost exclusively adenylate cyclase ( 19-21) and have been found in lung, liver, prostate gland, and seminal vesicles.	bind
22800	13	7217	6	13	NULL	NULL	NULL	VPAC2 receptor	GP		is found in					prostate gland	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_26_23562_s_31	11320087	2) VPAC1 and VPAC2 receptors, which bind both vasoactive intestinal polypeptide and PACAP but activate almost exclusively adenylate cyclase ( 19-21) and have been found in lung, liver, prostate gland, and seminal vesicles.	bind
22801	14	7217	6	13	NULL	NULL	NULL	VPAC2 receptor	GP		is found in					seminal vesicle	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_26_23562_s_31	11320087	2) VPAC1 and VPAC2 receptors, which bind both vasoactive intestinal polypeptide and PACAP but activate almost exclusively adenylate cyclase ( 19-21) and have been found in lung, liver, prostate gland, and seminal vesicles.	bind
27662	1	7217	7	10	NULL	0	NULL	VPAC1 receptors	NULL		bind	NULL				vasoactive intestinal polypeptide	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_26_23562_s_31	11320087	2) VPAC1 and VPAC2 receptors, which bind both vasoactive intestinal polypeptide and PACAP but activate almost exclusively adenylate cyclase ( 19-21) and have been found in lung, liver, prostate gland, and seminal vesicles.	bind
27663	2	7217	7	10	NULL	0	NULL	VPAC2 receptors	NULL		bind	NULL				vasoactive intestinal polypeptide	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_26_23562_s_31	11320087	2) VPAC1 and VPAC2 receptors, which bind both vasoactive intestinal polypeptide and PACAP but activate almost exclusively adenylate cyclase ( 19-21) and have been found in lung, liver, prostate gland, and seminal vesicles.	bind
27664	3	7217	7	10	NULL	0	NULL	VPAC1 receptors	NULL		bind	NULL				PACAP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_26_23562_s_31	11320087	2) VPAC1 and VPAC2 receptors, which bind both vasoactive intestinal polypeptide and PACAP but activate almost exclusively adenylate cyclase ( 19-21) and have been found in lung, liver, prostate gland, and seminal vesicles.	bind
27666	4	7217	7	10	NULL	0	NULL	VPAC2 receptors	NULL		bind	NULL				PACAP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_26_23562_s_31	11320087	2) VPAC1 and VPAC2 receptors, which bind both vasoactive intestinal polypeptide and PACAP but activate almost exclusively adenylate cyclase ( 19-21) and have been found in lung, liver, prostate gland, and seminal vesicles.	bind
27668	5	7217	7	10	NULL	0	NULL	VPAC1 receptor			activate		exclusively			adenylate cyclase					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_26_23562_s_31	11320087	2) VPAC1 and VPAC2 receptors, which bind both vasoactive intestinal polypeptide and PACAP but activate almost exclusively adenylate cyclase ( 19-21) and have been found in lung, liver, prostate gland, and seminal vesicles.	bind
27669	6	7217	7	10	NULL	0	NULL	VPAC2 receptor			activate		exclusively			adenylate cyclase					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_26_23562_s_31	11320087	2) VPAC1 and VPAC2 receptors, which bind both vasoactive intestinal polypeptide and PACAP but activate almost exclusively adenylate cyclase ( 19-21) and have been found in lung, liver, prostate gland, and seminal vesicles.	bind
27670	7	7217	7	10	NULL	0	NULL	VPAC1 receptor			is found in					lung					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_26_23562_s_31	11320087	2) VPAC1 and VPAC2 receptors, which bind both vasoactive intestinal polypeptide and PACAP but activate almost exclusively adenylate cyclase ( 19-21) and have been found in lung, liver, prostate gland, and seminal vesicles.	bind
27672	8	7217	7	10	NULL	0	NULL	VPAC1 receptor			is found in					liver					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_26_23562_s_31	11320087	2) VPAC1 and VPAC2 receptors, which bind both vasoactive intestinal polypeptide and PACAP but activate almost exclusively adenylate cyclase ( 19-21) and have been found in lung, liver, prostate gland, and seminal vesicles.	bind
54112	9	7217	7	10	NULL	0	NULL	VPAC1 receptor			is found in					prostate gland					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_26_23562_s_31	11320087	2) VPAC1 and VPAC2 receptors, which bind both vasoactive intestinal polypeptide and PACAP but activate almost exclusively adenylate cyclase ( 19-21) and have been found in lung, liver, prostate gland, and seminal vesicles.	bind
54113	10	7217	7	10	NULL	0	NULL	VPAC1 receptor			is found in					seminal vesicles					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_26_23562_s_31	11320087	2) VPAC1 and VPAC2 receptors, which bind both vasoactive intestinal polypeptide and PACAP but activate almost exclusively adenylate cyclase ( 19-21) and have been found in lung, liver, prostate gland, and seminal vesicles.	bind
54114	11	7217	7	10	NULL	0	NULL	VPAC2 receptor			is found in					lung					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_26_23562_s_31	11320087	2) VPAC1 and VPAC2 receptors, which bind both vasoactive intestinal polypeptide and PACAP but activate almost exclusively adenylate cyclase ( 19-21) and have been found in lung, liver, prostate gland, and seminal vesicles.	bind
54115	12	7217	7	10	NULL	0	NULL	VPAC2 receptor			is found in					liver					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_26_23562_s_31	11320087	2) VPAC1 and VPAC2 receptors, which bind both vasoactive intestinal polypeptide and PACAP but activate almost exclusively adenylate cyclase ( 19-21) and have been found in lung, liver, prostate gland, and seminal vesicles.	bind
54116	13	7217	7	10	NULL	0	NULL	VPAC2 receptor			is found in					prostate gland					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_26_23562_s_31	11320087	2) VPAC1 and VPAC2 receptors, which bind both vasoactive intestinal polypeptide and PACAP but activate almost exclusively adenylate cyclase ( 19-21) and have been found in lung, liver, prostate gland, and seminal vesicles.	bind
54117	14	7217	7	10	NULL	0	NULL	VPAC2 receptor			is found in					seminal vesicles					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_26_23562_s_31	11320087	2) VPAC1 and VPAC2 receptors, which bind both vasoactive intestinal polypeptide and PACAP but activate almost exclusively adenylate cyclase ( 19-21) and have been found in lung, liver, prostate gland, and seminal vesicles.	bind
22933	1	7221	6	13	NULL	NULL	NULL	apoB gene	GP		increase				LDLR binding region	LDL cholesterol	Chemical	levels of 			NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_34_0_233_s_110	11092828	2), in familial hypercholesterolemia,  and the LDLR binding region of the apo B gene (chromosome 2p23-p24), in familial  defective apo B100, have both been shown to increase LDL cholesterol levels and risk  of coronary heart disease ( 34,  40,  47,  67,  85,  101).	bind
22934	2	7221	6	13	NULL	NULL	NULL	statement 1	Process		occurs in					familial hypercholesterolemia	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_34_0_233_s_110	11092828	2), in familial hypercholesterolemia,  and the LDLR binding region of the apo B gene (chromosome 2p23-p24), in familial  defective apo B100, have both been shown to increase LDL cholesterol levels and risk  of coronary heart disease ( 34,  40,  47,  67,  85,  101).	bind
22935	3	7221	6	13	NULL	NULL	NULL	apoB-100	GP	defective	increases					LDL cholesterol	Chemical	levels of			NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_34_0_233_s_110	11092828	2), in familial hypercholesterolemia,  and the LDLR binding region of the apo B gene (chromosome 2p23-p24), in familial  defective apo B100, have both been shown to increase LDL cholesterol levels and risk  of coronary heart disease ( 34,  40,  47,  67,  85,  101).	bind
22936	4	7221	6	13	NULL	NULL	NULL	statement 3	Process		occurs in					familial hypercholesterolemia	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_34_0_233_s_110	11092828	2), in familial hypercholesterolemia,  and the LDLR binding region of the apo B gene (chromosome 2p23-p24), in familial  defective apo B100, have both been shown to increase LDL cholesterol levels and risk  of coronary heart disease ( 34,  40,  47,  67,  85,  101).	bind
22937	5	7221	6	13	NULL	NULL	NULL	apoB gene	GP		increases				LDLR binding region	coronary heart disease	MedicalFinding	risk of			NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_34_0_233_s_110	11092828	2), in familial hypercholesterolemia,  and the LDLR binding region of the apo B gene (chromosome 2p23-p24), in familial  defective apo B100, have both been shown to increase LDL cholesterol levels and risk  of coronary heart disease ( 34,  40,  47,  67,  85,  101).	bind
22938	6	7221	6	13	NULL	NULL	NULL	apoB-100	GP	defective	increases					coronary heart disease	MedicalFinding	risk of			NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_34_0_233_s_110	11092828	2), in familial hypercholesterolemia,  and the LDLR binding region of the apo B gene (chromosome 2p23-p24), in familial  defective apo B100, have both been shown to increase LDL cholesterol levels and risk  of coronary heart disease ( 34,  40,  47,  67,  85,  101).	bind
27853	1	7221	7	NULL	NULL	0	NULL	apoB gene	NULL		increase	NULL			LDLR binding region 	LDL cholesterol	NULL	levels of			NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_34_0_233_s_110	11092828	2), in familial hypercholesterolemia,  and the LDLR binding region of the apo B gene (chromosome 2p23-p24), in familial  defective apo B100, have both been shown to increase LDL cholesterol levels and risk  of coronary heart disease ( 34,  40,  47,  67,  85,  101).	bind
27854	2	7221	7	NULL	NULL	0	NULL	 apo B100	NULL	familial defective	increase	NULL				LDL cholesterol	NULL	levels of			NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_34_0_233_s_110	11092828	2), in familial hypercholesterolemia,  and the LDLR binding region of the apo B gene (chromosome 2p23-p24), in familial  defective apo B100, have both been shown to increase LDL cholesterol levels and risk  of coronary heart disease ( 34,  40,  47,  67,  85,  101).	bind
27855	3	7221	7	NULL	NULL	0	NULL	statement 1	NULL		increase	NULL				coronary heart disease	NULL	risk of			NULL		0	NULL	NULL	NULL	gw70_annurevgenet_34_0_233_s_110	11092828	2), in familial hypercholesterolemia,  and the LDLR binding region of the apo B gene (chromosome 2p23-p24), in familial  defective apo B100, have both been shown to increase LDL cholesterol levels and risk  of coronary heart disease ( 34,  40,  47,  67,  85,  101).	bind
27856	4	7221	7	NULL	NULL	0	NULL	statement 2	NULL		increase	NULL				coronary heart disease	NULL	risk of			NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_34_0_233_s_110	11092828	2), in familial hypercholesterolemia,  and the LDLR binding region of the apo B gene (chromosome 2p23-p24), in familial  defective apo B100, have both been shown to increase LDL cholesterol levels and risk  of coronary heart disease ( 34,  40,  47,  67,  85,  101).	bind
27866	5	7221	7	NULL	NULL	0	NULL	statement 1	NULL		occurs in	NULL				familial hypercholesterolemia	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevgenet_34_0_233_s_110	11092828	2), in familial hypercholesterolemia,  and the LDLR binding region of the apo B gene (chromosome 2p23-p24), in familial  defective apo B100, have both been shown to increase LDL cholesterol levels and risk  of coronary heart disease ( 34,  40,  47,  67,  85,  101).	bind
22803	1	7224	6	13	NULL	NULL	NULL	AGS3	GP		bind		preferentially			Galpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_43_33193_s_22	10969064	2, 3 AGS3 preferentially binds to Galpha in the presence of GDP ( 1).	bind
22804	2	7224	6	13	NULL	NULL	NULL	statement 1	Process		occurs in presence of					GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_43_33193_s_22	10969064	2, 3 AGS3 preferentially binds to Galpha in the presence of GDP ( 1).	bind
27679	1	7224	7	NULL	NULL	0	NULL	AGS3	NULL		binds	NULL	preferentially			Galpha	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_43_33193_s_22	10969064	2, 3 AGS3 preferentially binds to Galpha in the presence of GDP ( 1).	bind
27680	2	7224	7	NULL	NULL	0	NULL	statement 1	NULL		in presence of	NULL				GDP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_43_33193_s_22	10969064	2, 3 AGS3 preferentially binds to Galpha in the presence of GDP ( 1).	bind
22805	1	7225	6	13	NULL	NULL	NULL	emerin	GP		bind					multiple transcription factors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_6969_s_239	12493765	2, 3 We therefore suggest that EDMD disease results from the combined loss of emerin binding to multiple transcription factors, some of which may be more "`important"` than others in maintaining the function of a specific tissue.	bind
22806	2	7225	6	13	NULL	NULL	NULL	statement 1	Process	combined loss of	results in					EDMD disease	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_6969_s_239	12493765	2, 3 We therefore suggest that EDMD disease results from the combined loss of emerin binding to multiple transcription factors, some of which may be more "`important"` than others in maintaining the function of a specific tissue.	bind
27681	1	7225	7	NULL	NULL	0	NULL	emerin	NULL		bind	NULL				multiple transcription factors	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_9_6969_s_239	12493765	2, 3 We therefore suggest that EDMD disease results from the combined loss of emerin binding to multiple transcription factors, some of which may be more "`important"` than others in maintaining the function of a specific tissue.	bind
53627	2	7225	7	10	NULL	0	NULL	statement 1	NULL	combined loss of	results in	NULL				EDMD disease	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_9_6969_s_239	12493765	2, 3 We therefore suggest that EDMD disease results from the combined loss of emerin binding to multiple transcription factors, some of which may be more "`important"` than others in maintaining the function of a specific tissue.	bind
22807	1	7226	6	13	NULL	NULL	NULL	SHP2	GP		bind			SH2 domain		tyrosine kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_7_1081_s_103	12117720	2, 3, 14 SHP2 binds to tyrosine kinases via its SH2 domains and is activated by phosphorylation of its tyrosine residue.	bind
22808	2	7226	6	13	NULL	NULL	NULL	SHP2	GP		is activated by					SHP2	GP	phosphorylation of	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_7_1081_s_103	12117720	2, 3, 14 SHP2 binds to tyrosine kinases via its SH2 domains and is activated by phosphorylation of its tyrosine residue.	bind
27682	1	7226	7	10	NULL	0	NULL	 SHP2	NULL		binds	NULL		SH2 domain		tyrosine kinase	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_7_1081_s_103	12117720	2, 3, 14 SHP2 binds to tyrosine kinases via its SH2 domains and is activated by phosphorylation of its tyrosine residue.	bind
27683	2	7226	7	NULL	NULL	0	NULL		NULL	phosphorylation of	activates	NULL		tyrosine residue		tyrosine kinase	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_7_1081_s_103	12117720	2, 3, 14 SHP2 binds to tyrosine kinases via its SH2 domains and is activated by phosphorylation of its tyrosine residue.	bind
22809	1	7227	6	13	NULL	NULL	NULL	statement 3	GP		interacts with		electrostatically			statement 4	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_48_50150_s_266	15328339	2, at the initial low ratio of S3:LPS, binding of S3 dimer to LPS occurs via ( a) electrostatic interactions between the positively charged amino acid residues near  the N termini of S3 dimer and the negatively charged bisphosphate head groups of  the lipid A moiety of LPS and ( b) hydrophobic interactions between the C termini of S3 dimer and the acyl chains of  lipid A.	bind
22939	2	7227	6	13	NULL	NULL	NULL	S3 dimer	GP		interacts with		hydrophobically 	C termini		LPS	Chemical		acyl chains of lipid A		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_48_50150_s_266	15328339	2, at the initial low ratio of S3:LPS, binding of S3 dimer to LPS occurs via ( a) electrostatic interactions between the positively charged amino acid residues near  the N termini of S3 dimer and the negatively charged bisphosphate head groups of  the lipid A moiety of LPS and ( b) hydrophobic interactions between the C termini of S3 dimer and the acyl chains of  lipid A.	bind
53628	3	7227	6	13	NULL	NULL	NULL	S3 dimer	GP	positively charged amino acid	resides near					S3 dimer	GP		N termini		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_48_50150_s_266	15328339	2, at the initial low ratio of S3:LPS, binding of S3 dimer to LPS occurs via ( a) electrostatic interactions between the positively charged amino acid residues near  the N termini of S3 dimer and the negatively charged bisphosphate head groups of  the lipid A moiety of LPS and ( b) hydrophobic interactions between the C termini of S3 dimer and the acyl chains of  lipid A.	bind
53629	4	7227	6	13	NULL	NULL	NULL	LPS	Chemical		contains			lipid A moiety					negatively charged bisphosphate head groups		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_48_50150_s_266	15328339	2, at the initial low ratio of S3:LPS, binding of S3 dimer to LPS occurs via ( a) electrostatic interactions between the positively charged amino acid residues near  the N termini of S3 dimer and the negatively charged bisphosphate head groups of  the lipid A moiety of LPS and ( b) hydrophobic interactions between the C termini of S3 dimer and the acyl chains of  lipid A.	bind
27684	1	7227	7	NULL	NULL	0	NULL	S3 dimer	NULL		binds	NULL				LPS	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_50150_s_266	15328339	2, at the initial low ratio of S3:LPS, binding of S3 dimer to LPS occurs via ( a) electrostatic interactions between the positively charged amino acid residues near  the N termini of S3 dimer and the negatively charged bisphosphate head groups of  the lipid A moiety of LPS and ( b) hydrophobic interactions between the C termini of S3 dimer and the acyl chains of  lipid A.	bind
27685	2	7227	7	10	NULL	0	NULL	statement 5	NULL		interacts with	NULL	electrostatically			statement 6	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_48_50150_s_266	15328339	2, at the initial low ratio of S3:LPS, binding of S3 dimer to LPS occurs via ( a) electrostatic interactions between the positively charged amino acid residues near  the N termini of S3 dimer and the negatively charged bisphosphate head groups of  the lipid A moiety of LPS and ( b) hydrophobic interactions between the C termini of S3 dimer and the acyl chains of  lipid A.	bind
27686	3	7227	7	NULL	NULL	0	NULL	statement 1	NULL		occurs via	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_50150_s_266	15328339	2, at the initial low ratio of S3:LPS, binding of S3 dimer to LPS occurs via ( a) electrostatic interactions between the positively charged amino acid residues near  the N termini of S3 dimer and the negatively charged bisphosphate head groups of  the lipid A moiety of LPS and ( b) hydrophobic interactions between the C termini of S3 dimer and the acyl chains of  lipid A.	bind
27687	4	7227	7	10	NULL	0	NULL	S3 dimer	NULL		interacts with	NULL	hydrophobically	C termini of		lipid A	NULL		acyl chains of		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_48_50150_s_266	15328339	2, at the initial low ratio of S3:LPS, binding of S3 dimer to LPS occurs via ( a) electrostatic interactions between the positively charged amino acid residues near  the N termini of S3 dimer and the negatively charged bisphosphate head groups of  the lipid A moiety of LPS and ( b) hydrophobic interactions between the C termini of S3 dimer and the acyl chains of  lipid A.	bind
53630	5	7227	7	10	NULL	0	NULL	S3 dimer	NULL	\tpositively charged amino acid 	resides near	NULL				S3 dimer	NULL		N termini		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_50150_s_266	15328339	2, at the initial low ratio of S3:LPS, binding of S3 dimer to LPS occurs via ( a) electrostatic interactions between the positively charged amino acid residues near  the N termini of S3 dimer and the negatively charged bisphosphate head groups of  the lipid A moiety of LPS and ( b) hydrophobic interactions between the C termini of S3 dimer and the acyl chains of  lipid A.	bind
53631	6	7227	7	10	NULL	0	NULL	LPS	NULL		contains	NULL		lipid A moiety			NULL		negatively charged bisphosphate head groups		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_50150_s_266	15328339	2, at the initial low ratio of S3:LPS, binding of S3 dimer to LPS occurs via ( a) electrostatic interactions between the positively charged amino acid residues near  the N termini of S3 dimer and the negatively charged bisphosphate head groups of  the lipid A moiety of LPS and ( b) hydrophobic interactions between the C termini of S3 dimer and the acyl chains of  lipid A.	bind
22810	1	7228	6	13	NULL	NULL	NULL	ATP	Chemical		bind					P2X receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_20_23_8868_s_240	11102496	2, ATP binds to the P2X receptor resulting in the opening of a nonspecific ion channel.	bind
22811	2	7228	6	13	NULL	NULL	NULL	statement 1	Process		results in					nonspecific ion channel	Process	opening of 			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_20_23_8868_s_240	11102496	2, ATP binds to the P2X receptor resulting in the opening of a nonspecific ion channel.	bind
27688	1	7228	7	NULL	NULL	0	NULL	ATP 	NULL		binds to	NULL				P2X receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_23_8868_s_240	11102496	2, ATP binds to the P2X receptor resulting in the opening of a nonspecific ion channel.	bind
27689	2	7228	7	10	NULL	0	NULL	statement 1	NULL		results in	NULL				nonspecific ion channel	NULL	opening of			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_20_23_8868_s_240	11102496	2, ATP binds to the P2X receptor resulting in the opening of a nonspecific ion channel.	bind
22812	1	7229	6	13	NULL	NULL	NULL	heparin	Chemical	biotin-labeled	bind					Tg	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_18_12898_s_210	10212279	2, binding of biotin-labeled heparin to Tg-coated wells in the presence of 500 units/ml of unlabeled heparin.	bind
22813	2	7229	6	13	NULL	NULL	NULL	statement 1	Process		occurs in presence of					heparin	Chemical	unlabeled			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_18_12898_s_210	10212279	2, binding of biotin-labeled heparin to Tg-coated wells in the presence of 500 units/ml of unlabeled heparin.	bind
27690	1	7229	7	10	NULL	0	NULL	heparin	NULL	biotin-labeled 	binds to	NULL				Tg	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_18_12898_s_210	10212279	2, binding of biotin-labeled heparin to Tg-coated wells in the presence of 500 units/ml of unlabeled heparin.	bind
27691	2	7229	7	NULL	NULL	0	NULL	statement 1	NULL		in presence of	NULL				heparin	NULL	unlabeled			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_18_12898_s_210	10212279	2, binding of biotin-labeled heparin to Tg-coated wells in the presence of 500 units/ml of unlabeled heparin.	bind
22814	1	7230	6	13	NULL	NULL	NULL	Rifampin	Chemical		bind					RNAP	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_41_14925_s_130	15466710	2, Certain mutations (asterisks) on the  rpoB gene diminish the binding of rifampin to RNAP, making bacteria resistant in the presence  of rifampin.	bind
22815	2	7230	6	13	NULL	NULL	NULL	rpoB gene	GP	mutant	diminish					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_41_14925_s_130	15466710	2, Certain mutations (asterisks) on the  rpoB gene diminish the binding of rifampin to RNAP, making bacteria resistant in the presence  of rifampin.	bind
22816	3	7230	6	13	NULL	NULL	NULL	statement 1	Process		make					resistant bacteria	Organism				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_41_14925_s_130	15466710	2, Certain mutations (asterisks) on the  rpoB gene diminish the binding of rifampin to RNAP, making bacteria resistant in the presence  of rifampin.	bind
22817	4	7230	6	13	NULL	NULL	NULL	statement 3	Process		occurs in presence of					rifampin	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_41_14925_s_130	15466710	2, Certain mutations (asterisks) on the  rpoB gene diminish the binding of rifampin to RNAP, making bacteria resistant in the presence  of rifampin.	bind
27692	1	7230	7	NULL	NULL	0	NULL	rifampin	NULL		bind	NULL				RNAP	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_101_41_14925_s_130	15466710	2, Certain mutations (asterisks) on the  rpoB gene diminish the binding of rifampin to RNAP, making bacteria resistant in the presence  of rifampin.	bind
27693	2	7230	7	NULL	NULL	0	NULL	 rpoB gene	NULL	mutant	diminish	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_101_41_14925_s_130	15466710	2, Certain mutations (asterisks) on the  rpoB gene diminish the binding of rifampin to RNAP, making bacteria resistant in the presence  of rifampin.	bind
27694	3	7230	7	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				bacteria	NULL	resistance of			NULL		0	NULL	NULL	NULL	gw70_pnas_101_41_14925_s_130	15466710	2, Certain mutations (asterisks) on the  rpoB gene diminish the binding of rifampin to RNAP, making bacteria resistant in the presence  of rifampin.	bind
27695	4	7230	7	NULL	NULL	0	NULL	statement 3	NULL		in the presence of	NULL				rifampin	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_101_41_14925_s_130	15466710	2, Certain mutations (asterisks) on the  rpoB gene diminish the binding of rifampin to RNAP, making bacteria resistant in the presence  of rifampin.	bind
22818	1	7231	6	13	NULL	NULL	NULL	Tau	GP		bind					MT surface	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_30335_s_337	10869348	2, initial binding of Tau to the MT surface (first phase of binding), accompanied by a conformational change.	bind
27872	1	7231	7	NULL	NULL	0	NULL	Tau 	NULL		bind	NULL				MT surface	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_39_30335_s_337	10869348	2, initial binding of Tau to the MT surface (first phase of binding), accompanied by a conformational change.	bind
27873	2	7231	7	NULL	NULL	0	NULL	conformational change	NULL		accompanies	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_39_30335_s_337	10869348	2, initial binding of Tau to the MT surface (first phase of binding), accompanied by a conformational change.	bind
22819	1	7232	6	13	NULL	NULL	NULL	Hb:Hp ligand	GP		bind					CD163	GP				NULL	human monocyte-macrophages isolated in vitro	NULL	NULL	NULL	NULL	gw70_circulationres_94_1_119_s_163	14656926	2,19 - 22     In this study we demonstrate for the first time that Hb:Hp ligand binding to CD163 on human monocyte-macrophages isolated in vitro and in vivo elicits a direct antiinflammatory effect via the secretion of IL-10.	bind
22940	2	7232	6	13	NULL	NULL	NULL	Hb:Hp ligand	GP		bind					CD163	GP				NULL	human monocyte-macrophages isolated in vivo	NULL	NULL	NULL	NULL	gw70_circulationres_94_1_119_s_163	14656926	2,19 - 22     In this study we demonstrate for the first time that Hb:Hp ligand binding to CD163 on human monocyte-macrophages isolated in vitro and in vivo elicits a direct antiinflammatory effect via the secretion of IL-10.	bind
22941	3	7232	6	13	NULL	NULL	NULL	statement 1	Process		elicits					antiinflammatory response	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_1_119_s_163	14656926	2,19 - 22     In this study we demonstrate for the first time that Hb:Hp ligand binding to CD163 on human monocyte-macrophages isolated in vitro and in vivo elicits a direct antiinflammatory effect via the secretion of IL-10.	bind
22942	4	7232	6	13	NULL	NULL	NULL	statement 2	Process		elicits					antiinflammatory response	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_1_119_s_163	14656926	2,19 - 22     In this study we demonstrate for the first time that Hb:Hp ligand binding to CD163 on human monocyte-macrophages isolated in vitro and in vivo elicits a direct antiinflammatory effect via the secretion of IL-10.	bind
22943	5	7232	6	13	NULL	NULL	NULL	statement 3	Process		occurs via					IL-10	GP	secretion of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_1_119_s_163	14656926	2,19 - 22     In this study we demonstrate for the first time that Hb:Hp ligand binding to CD163 on human monocyte-macrophages isolated in vitro and in vivo elicits a direct antiinflammatory effect via the secretion of IL-10.	bind
22944	6	7232	6	13	NULL	NULL	NULL	statement 4	Process		occurs via					IL-10	GP	secretion of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_1_119_s_163	14656926	2,19 - 22     In this study we demonstrate for the first time that Hb:Hp ligand binding to CD163 on human monocyte-macrophages isolated in vitro and in vivo elicits a direct antiinflammatory effect via the secretion of IL-10.	bind
27875	1	7232	7	NULL	NULL	0	NULL	Hb:Hp ligand	NULL		bind	NULL				CD163	NULL	human			NULL	monocyte-macrophages in vitro	NULL	NULL	NULL	NULL	gw70_circulationres_94_1_119_s_163	14656926	2,19 - 22     In this study we demonstrate for the first time that Hb:Hp ligand binding to CD163 on human monocyte-macrophages isolated in vitro and in vivo elicits a direct antiinflammatory effect via the secretion of IL-10.	bind
27876	2	7232	7	NULL	NULL	0	NULL	Hb:Hp ligand	NULL		bind	NULL				CD163	NULL	human			NULL	 monocyte-macrophages in vivo	NULL	NULL	NULL	NULL	gw70_circulationres_94_1_119_s_163	14656926	2,19 - 22     In this study we demonstrate for the first time that Hb:Hp ligand binding to CD163 on human monocyte-macrophages isolated in vitro and in vivo elicits a direct antiinflammatory effect via the secretion of IL-10.	bind
27879	3	7232	7	NULL	NULL	0	NULL	statement 1	NULL		elicits	NULL				antiinflammatory effect 	NULL	direct			NULL		0	NULL	NULL	NULL	gw70_circulationres_94_1_119_s_163	14656926	2,19 - 22     In this study we demonstrate for the first time that Hb:Hp ligand binding to CD163 on human monocyte-macrophages isolated in vitro and in vivo elicits a direct antiinflammatory effect via the secretion of IL-10.	bind
27880	4	7232	7	NULL	NULL	0	NULL	statement 2	NULL		elicits	NULL				antiinflammatory effect 	NULL	direct			NULL		0	NULL	NULL	NULL	gw70_circulationres_94_1_119_s_163	14656926	2,19 - 22     In this study we demonstrate for the first time that Hb:Hp ligand binding to CD163 on human monocyte-macrophages isolated in vitro and in vivo elicits a direct antiinflammatory effect via the secretion of IL-10.	bind
27882	5	7232	7	NULL	NULL	0	NULL	statement 3	NULL		occurs via	NULL				IL-10	NULL	secretion of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_1_119_s_163	14656926	2,19 - 22     In this study we demonstrate for the first time that Hb:Hp ligand binding to CD163 on human monocyte-macrophages isolated in vitro and in vivo elicits a direct antiinflammatory effect via the secretion of IL-10.	bind
27883	6	7232	7	NULL	NULL	0	NULL	statement 4	NULL		occurs via	NULL				IL-10	NULL	secretion of			NULL		0	NULL	NULL	NULL	gw70_circulationres_94_1_119_s_163	14656926	2,19 - 22     In this study we demonstrate for the first time that Hb:Hp ligand binding to CD163 on human monocyte-macrophages isolated in vitro and in vivo elicits a direct antiinflammatory effect via the secretion of IL-10.	bind
22820	1	7233	6	13	NULL	NULL	NULL	cholesterol	Chemical		bind					(apo)B-containing lipoproteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_9_1972_s_25	15994445	2,3  In FLD, plasma LCAT is either absent or completely lacks catalytic activity; in FED, the mutant LCAT lacks activity on HDL lipids but esterifies cholesterol bound to apolipoprotein (apo)B-containing lipoproteins.	bind
22945	2	7233	6	13	NULL	NULL	NULL	plasma LCAT	GP		completely lacks					catalytic activity	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_9_1972_s_25	15994445	2,3  In FLD, plasma LCAT is either absent or completely lacks catalytic activity; in FED, the mutant LCAT lacks activity on HDL lipids but esterifies cholesterol bound to apolipoprotein (apo)B-containing lipoproteins.	bind
22946	3	7233	6	13	NULL	NULL	NULL	statement 2	Process		occurs in					FLD	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_9_1972_s_25	15994445	2,3  In FLD, plasma LCAT is either absent or completely lacks catalytic activity; in FED, the mutant LCAT lacks activity on HDL lipids but esterifies cholesterol bound to apolipoprotein (apo)B-containing lipoproteins.	bind
22947	4	7233	6	13	NULL	NULL	NULL	LCAT	GP	mutant	lacks activity on					HDL lipids	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_9_1972_s_25	15994445	2,3  In FLD, plasma LCAT is either absent or completely lacks catalytic activity; in FED, the mutant LCAT lacks activity on HDL lipids but esterifies cholesterol bound to apolipoprotein (apo)B-containing lipoproteins.	bind
22948	5	7233	6	13	NULL	NULL	NULL	LCAT	GP	mutant	esterifies					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_9_1972_s_25	15994445	2,3  In FLD, plasma LCAT is either absent or completely lacks catalytic activity; in FED, the mutant LCAT lacks activity on HDL lipids but esterifies cholesterol bound to apolipoprotein (apo)B-containing lipoproteins.	bind
22949	6	7233	6	13	NULL	NULL	NULL	statement 4	Process		occurs in					FED	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_9_1972_s_25	15994445	2,3  In FLD, plasma LCAT is either absent or completely lacks catalytic activity; in FED, the mutant LCAT lacks activity on HDL lipids but esterifies cholesterol bound to apolipoprotein (apo)B-containing lipoproteins.	bind
22950	7	7233	6	13	NULL	NULL	NULL	statement 5	Process		occurs in					FED	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_9_1972_s_25	15994445	2,3  In FLD, plasma LCAT is either absent or completely lacks catalytic activity; in FED, the mutant LCAT lacks activity on HDL lipids but esterifies cholesterol bound to apolipoprotein (apo)B-containing lipoproteins.	bind
27887	1	7233	7	NULL	NULL	0	NULL	LCAT	NULL		lacks 	NULL				catalytic activity	NULL				NULL	FLD	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_9_1972_s_25	15994445	2,3  In FLD, plasma LCAT is either absent or completely lacks catalytic activity; in FED, the mutant LCAT lacks activity on HDL lipids but esterifies cholesterol bound to apolipoprotein (apo)B-containing lipoproteins.	bind
27888	2	7233	7	NULL	NULL	0	NULL	LCAT	NULL	mutant	lacks	NULL				HDL lipids	NULL	activity on			NULL	FED	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_9_1972_s_25	15994445	2,3  In FLD, plasma LCAT is either absent or completely lacks catalytic activity; in FED, the mutant LCAT lacks activity on HDL lipids but esterifies cholesterol bound to apolipoprotein (apo)B-containing lipoproteins.	bind
27889	3	7233	7	NULL	NULL	0	NULL	cholesterol 	NULL		bind	NULL				(apo)B-containing lipoproteins	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_9_1972_s_25	15994445	2,3  In FLD, plasma LCAT is either absent or completely lacks catalytic activity; in FED, the mutant LCAT lacks activity on HDL lipids but esterifies cholesterol bound to apolipoprotein (apo)B-containing lipoproteins.	bind
27890	4	7233	7	NULL	NULL	0	NULL	LCAT	NULL	mutant	esterifies	NULL				statement 3	NULL				NULL	FED	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_9_1972_s_25	15994445	2,3  In FLD, plasma LCAT is either absent or completely lacks catalytic activity; in FED, the mutant LCAT lacks activity on HDL lipids but esterifies cholesterol bound to apolipoprotein (apo)B-containing lipoproteins.	bind
22821	1	7235	6	13	NULL	NULL	NULL	TCDD	Chemical		bind					Ah-R	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_52_1_30_s_2	9224809	2,3,7,8-Tetrachlorodibenzo-  p-dioxin (TCDD) binds and activates the aryl hydrocarbon receptor (Ah-R), an endogenous transcription factor that is expressed in the thymus.	bind
22822	2	7235	6	13	NULL	NULL	NULL	TCDD	Chemical		is					2,3,7,8-Tetrachlorodibenzo- p-dioxin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_52_1_30_s_2	9224809	2,3,7,8-Tetrachlorodibenzo-  p-dioxin (TCDD) binds and activates the aryl hydrocarbon receptor (Ah-R), an endogenous transcription factor that is expressed in the thymus.	bind
22823	3	7235	6	13	NULL	NULL	NULL	Ah-R	GP		is					aryl hydrocarbon receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_52_1_30_s_2	9224809	2,3,7,8-Tetrachlorodibenzo-  p-dioxin (TCDD) binds and activates the aryl hydrocarbon receptor (Ah-R), an endogenous transcription factor that is expressed in the thymus.	bind
22824	4	7235	6	13	NULL	NULL	NULL	Ah-R	GP		is a type of					transcription factor	GP	endogenous			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_52_1_30_s_2	9224809	2,3,7,8-Tetrachlorodibenzo-  p-dioxin (TCDD) binds and activates the aryl hydrocarbon receptor (Ah-R), an endogenous transcription factor that is expressed in the thymus.	bind
22825	5	7235	6	13	NULL	NULL	NULL	Ah-R	GP		is expressed in					thymus	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_52_1_30_s_2	9224809	2,3,7,8-Tetrachlorodibenzo-  p-dioxin (TCDD) binds and activates the aryl hydrocarbon receptor (Ah-R), an endogenous transcription factor that is expressed in the thymus.	bind
53632	6	7235	6	13	NULL	NULL	NULL	statement 1	Process		activates					Ah-R	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_52_1_30_s_2	9224809	2,3,7,8-Tetrachlorodibenzo-  p-dioxin (TCDD) binds and activates the aryl hydrocarbon receptor (Ah-R), an endogenous transcription factor that is expressed in the thymus.	bind
27892	1	7235	7	NULL	NULL	0	NULL	TCDD	NULL		binds	NULL				Ah-R	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_1_30_s_2	9224809	2,3,7,8-Tetrachlorodibenzo-  p-dioxin (TCDD) binds and activates the aryl hydrocarbon receptor (Ah-R), an endogenous transcription factor that is expressed in the thymus.	bind
27893	2	7235	7	10	NULL	0	NULL	statement 1	NULL		activates	NULL				Ah-R	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_52_1_30_s_2	9224809	2,3,7,8-Tetrachlorodibenzo-  p-dioxin (TCDD) binds and activates the aryl hydrocarbon receptor (Ah-R), an endogenous transcription factor that is expressed in the thymus.	bind
27895	3	7235	7	NULL	NULL	0	NULL	Ah-R	NULL		is a type of	NULL				transcription factor	NULL	endogenous			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_1_30_s_2	9224809	2,3,7,8-Tetrachlorodibenzo-  p-dioxin (TCDD) binds and activates the aryl hydrocarbon receptor (Ah-R), an endogenous transcription factor that is expressed in the thymus.	bind
27897	4	7235	7	NULL	NULL	0	NULL	Ah-R	NULL		is expressed in	NULL				thymus	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_1_30_s_2	9224809	2,3,7,8-Tetrachlorodibenzo-  p-dioxin (TCDD) binds and activates the aryl hydrocarbon receptor (Ah-R), an endogenous transcription factor that is expressed in the thymus.	bind
27898	5	7235	7	NULL	NULL	0	NULL	TCDD	NULL		is	NULL				2,3,7,8-Tetrachlorodibenzo- p-dioxin	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_1_30_s_2	9224809	2,3,7,8-Tetrachlorodibenzo-  p-dioxin (TCDD) binds and activates the aryl hydrocarbon receptor (Ah-R), an endogenous transcription factor that is expressed in the thymus.	bind
27900	6	7235	7	NULL	NULL	0	NULL	Ah-R	NULL		is	NULL				aryl hydrocarbon receptor	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_52_1_30_s_2	9224809	2,3,7,8-Tetrachlorodibenzo-  p-dioxin (TCDD) binds and activates the aryl hydrocarbon receptor (Ah-R), an endogenous transcription factor that is expressed in the thymus.	bind
22826	1	7237	6	13	NULL	NULL	NULL	DFA	Chemical		does not bind					hCyp-18	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_505_1_191_s_105	11557067	2,4-Difluoroaniline (DFA) did not bind hCyp-18.	bind
22827	2	7237	6	13	NULL	NULL	NULL	DFA	Chemical		is					2,4-Difluoroaniline 	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_505_1_191_s_105	11557067	2,4-Difluoroaniline (DFA) did not bind hCyp-18.	bind
27904	1	7237	7	NULL	NULL	0	NULL	DFA	NULL		does not bind	NULL				hCyp-18	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_505_1_191_s_105	11557067	2,4-Difluoroaniline (DFA) did not bind hCyp-18.	bind
27905	2	7237	7	NULL	NULL	0	NULL	DFA	NULL		is	NULL				2,4-Difluoroaniline	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_505_1_191_s_105	11557067	2,4-Difluoroaniline (DFA) did not bind hCyp-18.	bind
22951	1	7238	6	13	NULL	NULL	NULL	guanylate cyclase C receptor	GP		is					GC-C	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_6_2169_s_13	12466132	2- 4  Once elaborated into the intestinal lumen, guanylin, another similar mammalian peptide, uroguanylin, and STa can all bind to the receptor guanylate cyclase C (GC-C), located on the enterocyte brush border membrane.	bind
22952	2	7238	6	13	NULL	NULL	NULL	GC-C	GP		is located on					enterocyte brush border membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_6_2169_s_13	12466132	2- 4  Once elaborated into the intestinal lumen, guanylin, another similar mammalian peptide, uroguanylin, and STa can all bind to the receptor guanylate cyclase C (GC-C), located on the enterocyte brush border membrane.	bind
22953	3	7238	6	13	NULL	NULL	NULL	guanylin	GP		bind					GC-C	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_6_2169_s_13	12466132	2- 4  Once elaborated into the intestinal lumen, guanylin, another similar mammalian peptide, uroguanylin, and STa can all bind to the receptor guanylate cyclase C (GC-C), located on the enterocyte brush border membrane.	bind
22954	4	7238	6	13	NULL	NULL	NULL	uroguanylin	GP		bind					GC-C	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_6_2169_s_13	12466132	2- 4  Once elaborated into the intestinal lumen, guanylin, another similar mammalian peptide, uroguanylin, and STa can all bind to the receptor guanylate cyclase C (GC-C), located on the enterocyte brush border membrane.	bind
22955	5	7238	6	13	NULL	NULL	NULL	STa	GP		bind					GC-C	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_6_2169_s_13	12466132	2- 4  Once elaborated into the intestinal lumen, guanylin, another similar mammalian peptide, uroguanylin, and STa can all bind to the receptor guanylate cyclase C (GC-C), located on the enterocyte brush border membrane.	bind
27914	1	7238	7	NULL	NULL	0	NULL	guanylin	NULL		bind	NULL				GC-C receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_6_2169_s_13	12466132	2- 4  Once elaborated into the intestinal lumen, guanylin, another similar mammalian peptide, uroguanylin, and STa can all bind to the receptor guanylate cyclase C (GC-C), located on the enterocyte brush border membrane.	bind
27915	2	7238	7	NULL	NULL	0	NULL	uroguanylin	NULL		bind	NULL				receptor GC-C	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_6_2169_s_13	12466132	2- 4  Once elaborated into the intestinal lumen, guanylin, another similar mammalian peptide, uroguanylin, and STa can all bind to the receptor guanylate cyclase C (GC-C), located on the enterocyte brush border membrane.	bind
27916	3	7238	7	NULL	NULL	0	NULL	STa	NULL		bind	NULL				GC-C receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_6_2169_s_13	12466132	2- 4  Once elaborated into the intestinal lumen, guanylin, another similar mammalian peptide, uroguanylin, and STa can all bind to the receptor guanylate cyclase C (GC-C), located on the enterocyte brush border membrane.	bind
27917	4	7238	7	NULL	NULL	0	NULL	GC-C receptor	NULL		is located on the	NULL				enterocyte brush border membrane	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_6_2169_s_13	12466132	2- 4  Once elaborated into the intestinal lumen, guanylin, another similar mammalian peptide, uroguanylin, and STa can all bind to the receptor guanylate cyclase C (GC-C), located on the enterocyte brush border membrane.	bind
27918	5	7238	7	NULL	NULL	0	NULL	GC-C	NULL		is	NULL				guanylate cyclase C	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_6_2169_s_13	12466132	2- 4  Once elaborated into the intestinal lumen, guanylin, another similar mammalian peptide, uroguanylin, and STa can all bind to the receptor guanylate cyclase C (GC-C), located on the enterocyte brush border membrane.	bind
22848	1	7240	6	13	NULL	NULL	NULL	NF-kappaB	GP		bind					DNA	NucleicAcid				NULL	H4-II-E overproducing H9 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_1_413_s_210	11020383	2-AAF Activates NF-kappaB DNA Binding through Generating ROS-- Since mdr1b is a NF-kappaB-regulated gene and NF-kappaB is an important oxidative stress responder, we then compared 2-AAF induced NF-kappaB DNA binding activity in H4-II-E (Fig.  8 A) and GSH overproducing H9 cells (Fig.  8 B).	bind
22849	2	7240	6	13	NULL	NULL	NULL	AAF	Chemical		activates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_1_413_s_210	11020383	2-AAF Activates NF-kappaB DNA Binding through Generating ROS-- Since mdr1b is a NF-kappaB-regulated gene and NF-kappaB is an important oxidative stress responder, we then compared 2-AAF induced NF-kappaB DNA binding activity in H4-II-E (Fig.  8 A) and GSH overproducing H9 cells (Fig.  8 B).	bind
22850	3	7240	6	13	NULL	NULL	NULL	statement 1	Process		occurs through					ROS	GP	generation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_1_413_s_210	11020383	2-AAF Activates NF-kappaB DNA Binding through Generating ROS-- Since mdr1b is a NF-kappaB-regulated gene and NF-kappaB is an important oxidative stress responder, we then compared 2-AAF induced NF-kappaB DNA binding activity in H4-II-E (Fig.  8 A) and GSH overproducing H9 cells (Fig.  8 B).	bind
22851	4	7240	6	13	NULL	NULL	NULL	mdr1b gene	GP		is regulated by					NF-kappaB	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_1_413_s_210	11020383	2-AAF Activates NF-kappaB DNA Binding through Generating ROS-- Since mdr1b is a NF-kappaB-regulated gene and NF-kappaB is an important oxidative stress responder, we then compared 2-AAF induced NF-kappaB DNA binding activity in H4-II-E (Fig.  8 A) and GSH overproducing H9 cells (Fig.  8 B).	bind
22852	5	7240	6	13	NULL	NULL	NULL	NF-kappaB	GP		responds to					oxidative stress	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_1_413_s_210	11020383	2-AAF Activates NF-kappaB DNA Binding through Generating ROS-- Since mdr1b is a NF-kappaB-regulated gene and NF-kappaB is an important oxidative stress responder, we then compared 2-AAF induced NF-kappaB DNA binding activity in H4-II-E (Fig.  8 A) and GSH overproducing H9 cells (Fig.  8 B).	bind
22853	6	7240	6	13	NULL	NULL	NULL	NF-kappaB	GP		bind					DNA	NucleicAcid				NULL	GSH overproducing H9 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_1_413_s_210	11020383	2-AAF Activates NF-kappaB DNA Binding through Generating ROS-- Since mdr1b is a NF-kappaB-regulated gene and NF-kappaB is an important oxidative stress responder, we then compared 2-AAF induced NF-kappaB DNA binding activity in H4-II-E (Fig.  8 A) and GSH overproducing H9 cells (Fig.  8 B).	bind
22854	7	7240	6	13	NULL	NULL	NULL	AAF	Chemical		activates					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_1_413_s_210	11020383	2-AAF Activates NF-kappaB DNA Binding through Generating ROS-- Since mdr1b is a NF-kappaB-regulated gene and NF-kappaB is an important oxidative stress responder, we then compared 2-AAF induced NF-kappaB DNA binding activity in H4-II-E (Fig.  8 A) and GSH overproducing H9 cells (Fig.  8 B).	bind
53633	8	7240	6	13	NULL	NULL	NULL	AAF	Chemical		activates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_1_413_s_210	11020383	2-AAF Activates NF-kappaB DNA Binding through Generating ROS-- Since mdr1b is a NF-kappaB-regulated gene and NF-kappaB is an important oxidative stress responder, we then compared 2-AAF induced NF-kappaB DNA binding activity in H4-II-E (Fig.  8 A) and GSH overproducing H9 cells (Fig.  8 B).	bind
27919	1	7240	7	NULL	NULL	0	NULL	NF-kappaB	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_413_s_210	11020383	2-AAF Activates NF-kappaB DNA Binding through Generating ROS-- Since mdr1b is a NF-kappaB-regulated gene and NF-kappaB is an important oxidative stress responder, we then compared 2-AAF induced NF-kappaB DNA binding activity in H4-II-E (Fig.  8 A) and GSH overproducing H9 cells (Fig.  8 B).	bind
27920	2	7240	7	NULL	NULL	0	NULL	AAF	NULL		activates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_413_s_210	11020383	2-AAF Activates NF-kappaB DNA Binding through Generating ROS-- Since mdr1b is a NF-kappaB-regulated gene and NF-kappaB is an important oxidative stress responder, we then compared 2-AAF induced NF-kappaB DNA binding activity in H4-II-E (Fig.  8 A) and GSH overproducing H9 cells (Fig.  8 B).	bind
27921	3	7240	7	NULL	NULL	0	NULL	statement 2	NULL		occurs through	NULL				ROS	NULL	generating			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_413_s_210	11020383	2-AAF Activates NF-kappaB DNA Binding through Generating ROS-- Since mdr1b is a NF-kappaB-regulated gene and NF-kappaB is an important oxidative stress responder, we then compared 2-AAF induced NF-kappaB DNA binding activity in H4-II-E (Fig.  8 A) and GSH overproducing H9 cells (Fig.  8 B).	bind
27922	4	7240	7	NULL	NULL	0	NULL	NF-kappaB	NULL		regulates	NULL				 mdr1b gene	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_413_s_210	11020383	2-AAF Activates NF-kappaB DNA Binding through Generating ROS-- Since mdr1b is a NF-kappaB-regulated gene and NF-kappaB is an important oxidative stress responder, we then compared 2-AAF induced NF-kappaB DNA binding activity in H4-II-E (Fig.  8 A) and GSH overproducing H9 cells (Fig.  8 B).	bind
27923	5	7240	7	NULL	NULL	0	NULL	NF-kappaB	NULL		responds to	NULL				oxidative stress	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_413_s_210	11020383	2-AAF Activates NF-kappaB DNA Binding through Generating ROS-- Since mdr1b is a NF-kappaB-regulated gene and NF-kappaB is an important oxidative stress responder, we then compared 2-AAF induced NF-kappaB DNA binding activity in H4-II-E (Fig.  8 A) and GSH overproducing H9 cells (Fig.  8 B).	bind
27924	6	7240	7	NULL	NULL	0	NULL	AAF	NULL		induce	NULL				statement 1	NULL				NULL	H4-II-E overproducing H9 cells	0	NULL	NULL	NULL	gw60_jbiolchem_276_1_413_s_210	11020383	2-AAF Activates NF-kappaB DNA Binding through Generating ROS-- Since mdr1b is a NF-kappaB-regulated gene and NF-kappaB is an important oxidative stress responder, we then compared 2-AAF induced NF-kappaB DNA binding activity in H4-II-E (Fig.  8 A) and GSH overproducing H9 cells (Fig.  8 B).	bind
27925	7	7240	7	NULL	NULL	0	NULL	AAF	NULL		induce	NULL				statement 1	NULL				NULL	GSH overproducing H9 cells	0	NULL	NULL	NULL	gw60_jbiolchem_276_1_413_s_210	11020383	2-AAF Activates NF-kappaB DNA Binding through Generating ROS-- Since mdr1b is a NF-kappaB-regulated gene and NF-kappaB is an important oxidative stress responder, we then compared 2-AAF induced NF-kappaB DNA binding activity in H4-II-E (Fig.  8 A) and GSH overproducing H9 cells (Fig.  8 B).	bind
22855	1	7241	6	13	NULL	NULL	NULL	2-Acetoxyamino-6-methyldipyrido imidazole	Chemical		bind		covalently			DNA	NucleicAcid			guanine residues	NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochem-biophys-res-commun_116_3_6651841_s_2	6651841	2-Acetoxyamino-6-methyldipyrido[1,2-a:3'',2''-d]imidazole binds covalently  to the 8 position of guanine residues in DNA.	bind
27926	1	7241	7	NULL	NULL	0	NULL	2-Acetoxyamino-6-methyldipyrido[1,2-a:3'',2''-d]imidazole	NULL		binds	NULL	covalently			DNA	NULL			guanine residues	NULL		0	NULL	NULL	NULL	abs-batch0650-0679_biochem-biophys-res-commun_116_3_6651841_s_2	6651841	2-Acetoxyamino-6-methyldipyrido[1,2-a:3'',2''-d]imidazole binds covalently  to the 8 position of guanine residues in DNA.	bind
22856	1	7242	6	13	NULL	NULL	NULL	GTP	Chemical		bind					Rho	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevpharmacol_40_0_459_s_108	10836144	2-Adrenergic receptor stimulation increased [32]GTP binding to Rho and decreased [32]GDP-Rho binding in preadipocytes ( 52).	bind
22857	2	7242	6	13	NULL	NULL	NULL	Adrenergic receptor	GP	stimulation of	increases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevpharmacol_40_0_459_s_108	10836144	2-Adrenergic receptor stimulation increased [32]GTP binding to Rho and decreased [32]GDP-Rho binding in preadipocytes ( 52).	bind
22858	3	7242	6	13	NULL	NULL	NULL	GDP	Chemical		bind					Rho	GP				NULL	preadipocytes	NULL	NULL	NULL	NULL	gw70_annurevpharmacol_40_0_459_s_108	10836144	2-Adrenergic receptor stimulation increased [32]GTP binding to Rho and decreased [32]GDP-Rho binding in preadipocytes ( 52).	bind
22859	4	7242	6	13	NULL	NULL	NULL	Adrenergic receptor	GP	stimulation of	decreases					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevpharmacol_40_0_459_s_108	10836144	2-Adrenergic receptor stimulation increased [32]GTP binding to Rho and decreased [32]GDP-Rho binding in preadipocytes ( 52).	bind
27927	1	7242	7	10	NULL	0	NULL	GTP	NULL		bind	NULL				Rho	NULL				NULL		NULL	NULL	NULL	NULL	gw70_annurevpharmacol_40_0_459_s_108	10836144	2-Adrenergic receptor stimulation increased [32]GTP binding to Rho and decreased [32]GDP-Rho binding in preadipocytes ( 52).	bind
27928	2	7242	7	NULL	NULL	0	NULL	Adrenergic receptor	NULL	stimulation of	increase	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevpharmacol_40_0_459_s_108	10836144	2-Adrenergic receptor stimulation increased [32]GTP binding to Rho and decreased [32]GDP-Rho binding in preadipocytes ( 52).	bind
27929	3	7242	7	NULL	NULL	0	NULL	Adrenergic receptor	NULL	stimulation of	decrease	NULL				statement 1	NULL				NULL	preadipocytes	0	NULL	NULL	NULL	gw70_annurevpharmacol_40_0_459_s_108	10836144	2-Adrenergic receptor stimulation increased [32]GTP binding to Rho and decreased [32]GDP-Rho binding in preadipocytes ( 52).	bind
22860	1	7243	6	13	NULL	NULL	NULL	PPARgamma	GP		bind					PPAR	NucleicAcid			response element	NULL	activated Jurkat T cells	NULL	NULL	NULL	NULL	abs-batch0700-0719_mol-pharmacol_70_1_16611855_s_10	16611855	2-AG treatment  also induced PPARgamma binding to a PPAR response element in activated  Jurkat T cells.	bind
22861	2	7243	6	13	NULL	NULL	NULL	AG	Chemical	treatment with	induces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_mol-pharmacol_70_1_16611855_s_10	16611855	2-AG treatment  also induced PPARgamma binding to a PPAR response element in activated  Jurkat T cells.	bind
27930	1	7243	7	NULL	NULL	0	NULL	 PPARgamma	NULL		bind	NULL				PPAR	NULL			 response element	NULL	activated Jurkat T cells	0	NULL	NULL	NULL	abs-batch0700-0719_mol-pharmacol_70_1_16611855_s_10	16611855	2-AG treatment  also induced PPARgamma binding to a PPAR response element in activated  Jurkat T cells.	bind
27931	2	7243	7	10	NULL	0	NULL	AG	NULL	treatment	induce	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_mol-pharmacol_70_1_16611855_s_10	16611855	2-AG treatment  also induced PPARgamma binding to a PPAR response element in activated  Jurkat T cells.	bind
22862	1	7245	6	13	NULL	NULL	NULL	2-Chloro- cis,cis-muconate	Chemical		bind		high affinity			muconate cycloisomerase	GP	P. putida			NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_64_9_3290_s_205	9726873	2-Chloro- cis,cis-muconate binds to the  P. putida muconate cycloisomerase with a relatively high affinity but with a low  kcat (Table  3).	bind
27932	1	7245	7	NULL	NULL	0	NULL	2-Chloro- cis,cis-muconate	NULL		binds	NULL	high affinity			 muconate cycloisomerase	NULL	P. putida			NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_64_9_3290_s_205	9726873	2-Chloro- cis,cis-muconate binds to the  P. putida muconate cycloisomerase with a relatively high affinity but with a low  kcat (Table  3).	bind
22863	1	7246	6	13	NULL	NULL	NULL	2-Ketoglutarate	Chemical	C-labeled	bind					PII	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_30_17797_s_209	7629080	2-Ketoglutarate and ATP Bind to PII In order to  determine the target for 2-ketoglutarate, we used  C-labeled 2-ketoglutarate to measure directly the binding  of 2-ketoglutarate to the individual signal transduction components  (NRI, NRII, PII, and UTase/UR).	bind
22864	2	7246	6	13	NULL	NULL	NULL	ATP	Chemical		bind					PII	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_30_17797_s_209	7629080	2-Ketoglutarate and ATP Bind to PII In order to  determine the target for 2-ketoglutarate, we used  C-labeled 2-ketoglutarate to measure directly the binding  of 2-ketoglutarate to the individual signal transduction components  (NRI, NRII, PII, and UTase/UR).	bind
22865	3	7246	6	13	NULL	NULL	NULL	2-ketoglutarate	Chemical	C-labeled	bind					NRI	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_30_17797_s_209	7629080	2-Ketoglutarate and ATP Bind to PII In order to  determine the target for 2-ketoglutarate, we used  C-labeled 2-ketoglutarate to measure directly the binding  of 2-ketoglutarate to the individual signal transduction components  (NRI, NRII, PII, and UTase/UR).	bind
22866	4	7246	6	13	NULL	NULL	NULL	2-Ketoglutarate	Chemical	C-labeled	bind					NRII	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_30_17797_s_209	7629080	2-Ketoglutarate and ATP Bind to PII In order to  determine the target for 2-ketoglutarate, we used  C-labeled 2-ketoglutarate to measure directly the binding  of 2-ketoglutarate to the individual signal transduction components  (NRI, NRII, PII, and UTase/UR).	bind
22867	5	7246	6	13	NULL	NULL	NULL	2-Ketoglutarate	Chemical	C-labeled	bind					UTase/UR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_30_17797_s_209	7629080	2-Ketoglutarate and ATP Bind to PII In order to  determine the target for 2-ketoglutarate, we used  C-labeled 2-ketoglutarate to measure directly the binding  of 2-ketoglutarate to the individual signal transduction components  (NRI, NRII, PII, and UTase/UR).	bind
27933	1	7246	7	NULL	NULL	0	NULL	2-Ketoglutarate	NULL	C-labeled	bind	NULL				PII	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_30_17797_s_209	7629080	2-Ketoglutarate and ATP Bind to PII In order to  determine the target for 2-ketoglutarate, we used  C-labeled 2-ketoglutarate to measure directly the binding  of 2-ketoglutarate to the individual signal transduction components  (NRI, NRII, PII, and UTase/UR).	bind
27934	2	7246	7	NULL	NULL	0	NULL	 ATP	NULL		bind	NULL				PII	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_30_17797_s_209	7629080	2-Ketoglutarate and ATP Bind to PII In order to  determine the target for 2-ketoglutarate, we used  C-labeled 2-ketoglutarate to measure directly the binding  of 2-ketoglutarate to the individual signal transduction components  (NRI, NRII, PII, and UTase/UR).	bind
27936	4	7246	7	NULL	NULL	0	NULL	2-ketoglutarate	NULL	C-labeled	bind	NULL				NRI	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_30_17797_s_209	7629080	2-Ketoglutarate and ATP Bind to PII In order to  determine the target for 2-ketoglutarate, we used  C-labeled 2-ketoglutarate to measure directly the binding  of 2-ketoglutarate to the individual signal transduction components  (NRI, NRII, PII, and UTase/UR).	bind
27937	5	7246	7	NULL	NULL	0	NULL	2-ketoglutarate	NULL	C-labeled	bind	NULL				NRII	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_30_17797_s_209	7629080	2-Ketoglutarate and ATP Bind to PII In order to  determine the target for 2-ketoglutarate, we used  C-labeled 2-ketoglutarate to measure directly the binding  of 2-ketoglutarate to the individual signal transduction components  (NRI, NRII, PII, and UTase/UR).	bind
27938	6	7246	7	NULL	NULL	0	NULL	2-ketoglutarate	NULL	C-labeled	bind	NULL				UTase/UR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_30_17797_s_209	7629080	2-Ketoglutarate and ATP Bind to PII In order to  determine the target for 2-ketoglutarate, we used  C-labeled 2-ketoglutarate to measure directly the binding  of 2-ketoglutarate to the individual signal transduction components  (NRI, NRII, PII, and UTase/UR).	bind
22868	1	7247	6	13	NULL	NULL	NULL	2-Oxoglutarate	Chemical		bind					PII	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_8_2582_s_22	12670983	2-Oxoglutarate and ATP bind to PII in a synergistic manner ( ), stimulating the phosphorylation of  Synechococcus elongatus strain PCC 7942 PII at Ser 49 ( ,  ).	bind
22869	2	7247	6	13	NULL	NULL	NULL	ATP	Chemical		bind					PII	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_8_2582_s_22	12670983	2-Oxoglutarate and ATP bind to PII in a synergistic manner ( ), stimulating the phosphorylation of  Synechococcus elongatus strain PCC 7942 PII at Ser 49 ( ,  ).	bind
22870	3	7247	6	13	NULL	NULL	NULL	statement 1	Process		acts synergistically with 					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_8_2582_s_22	12670983	2-Oxoglutarate and ATP bind to PII in a synergistic manner ( ), stimulating the phosphorylation of  Synechococcus elongatus strain PCC 7942 PII at Ser 49 ( ,  ).	bind
22871	4	7247	6	13	NULL	NULL	NULL	statement 1	Process		stimulates					PCC 7942 PII	GP	phosphorylation of	Ser 49		NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_8_2582_s_22	12670983	2-Oxoglutarate and ATP bind to PII in a synergistic manner ( ), stimulating the phosphorylation of  Synechococcus elongatus strain PCC 7942 PII at Ser 49 ( ,  ).	bind
22872	5	7247	6	13	NULL	NULL	NULL	statement 2	Process		stimulates					PCC 7942 PII	GP	phosphorylation of	Ser 49		NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_8_2582_s_22	12670983	2-Oxoglutarate and ATP bind to PII in a synergistic manner ( ), stimulating the phosphorylation of  Synechococcus elongatus strain PCC 7942 PII at Ser 49 ( ,  ).	bind
46502	6	7247	6	13	NULL	NULL	NULL	PCC 7942 PII	Organism		is a strain of					Synechococcus elongatus	Organism				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_8_2582_s_22	12670983	2-Oxoglutarate and ATP bind to PII in a synergistic manner ( ), stimulating the phosphorylation of  Synechococcus elongatus strain PCC 7942 PII at Ser 49 ( ,  ).	bind
27939	1	7247	7	NULL	NULL	0	NULL	2-Oxoglutarate	NULL		bind	NULL				PII	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_8_2582_s_22	12670983	2-Oxoglutarate and ATP bind to PII in a synergistic manner ( ), stimulating the phosphorylation of  Synechococcus elongatus strain PCC 7942 PII at Ser 49 ( ,  ).	bind
27940	2	7247	7	NULL	NULL	0	NULL	ATP	NULL		bind	NULL				PII	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_8_2582_s_22	12670983	2-Oxoglutarate and ATP bind to PII in a synergistic manner ( ), stimulating the phosphorylation of  Synechococcus elongatus strain PCC 7942 PII at Ser 49 ( ,  ).	bind
27941	3	7247	7	NULL	NULL	0	NULL	statement 1	NULL		synergistically occur with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_8_2582_s_22	12670983	2-Oxoglutarate and ATP bind to PII in a synergistic manner ( ), stimulating the phosphorylation of  Synechococcus elongatus strain PCC 7942 PII at Ser 49 ( ,  ).	bind
27942	4	7247	7	10	NULL	0	NULL	statement 3	NULL		stimulate	NULL				PCC 7942 PII	NULL	phosphorylation of	Ser 49		NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_8_2582_s_22	12670983	2-Oxoglutarate and ATP bind to PII in a synergistic manner ( ), stimulating the phosphorylation of  Synechococcus elongatus strain PCC 7942 PII at Ser 49 ( ,  ).	bind
46503	5	7247	7	10	NULL	0	NULL	PCC 7942 PII	NULL		is a strain of	NULL				Synechococcus elongatus	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_8_2582_s_22	12670983	2-Oxoglutarate and ATP bind to PII in a synergistic manner ( ), stimulating the phosphorylation of  Synechococcus elongatus strain PCC 7942 PII at Ser 49 ( ,  ).	bind
22873	1	7249	6	13	NULL	NULL	NULL	PipX	GP		forms a complex with					NtcA	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_2_16796668_s_8	16796668	2-Oxoglutarate favours complex formation  between PipX and NtcA, but impairs binding to PII, suggesting that partner  swapping between these nitrogen regulators is driven by the 2-oxoglutarate  concentration.	bind
22874	2	7249	6	13	NULL	NULL	NULL	2-Oxoglutarate	Chemical		favours					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_2_16796668_s_8	16796668	2-Oxoglutarate favours complex formation  between PipX and NtcA, but impairs binding to PII, suggesting that partner  swapping between these nitrogen regulators is driven by the 2-oxoglutarate  concentration.	bind
22875	3	7249	6	13	NULL	NULL	NULL	PipX	GP		bind					PII	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_2_16796668_s_8	16796668	2-Oxoglutarate favours complex formation  between PipX and NtcA, but impairs binding to PII, suggesting that partner  swapping between these nitrogen regulators is driven by the 2-oxoglutarate  concentration.	bind
22876	4	7249	6	13	NULL	NULL	NULL	2-Oxoglutarate	Chemical		impairs					PII	GP	binding to			NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_2_16796668_s_8	16796668	2-Oxoglutarate favours complex formation  between PipX and NtcA, but impairs binding to PII, suggesting that partner  swapping between these nitrogen regulators is driven by the 2-oxoglutarate  concentration.	bind
46504	5	7249	6	13	NULL	NULL	NULL	PipX	GP		is a type of					nitrogen regulator	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_2_16796668_s_8	16796668	2-Oxoglutarate favours complex formation  between PipX and NtcA, but impairs binding to PII, suggesting that partner  swapping between these nitrogen regulators is driven by the 2-oxoglutarate  concentration.	bind
46505	6	7249	6	13	NULL	NULL	NULL	NtcA	GP		is a type of					nitrogen regulator	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_2_16796668_s_8	16796668	2-Oxoglutarate favours complex formation  between PipX and NtcA, but impairs binding to PII, suggesting that partner  swapping between these nitrogen regulators is driven by the 2-oxoglutarate  concentration.	bind
27943	1	7249	7	NULL	NULL	0	NULL	PipX	NULL		forms complex with	NULL				NtcA	NULL				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_2_16796668_s_8	16796668	2-Oxoglutarate favours complex formation  between PipX and NtcA, but impairs binding to PII, suggesting that partner  swapping between these nitrogen regulators is driven by the 2-oxoglutarate  concentration.	bind
27944	2	7249	7	NULL	NULL	0	NULL	2-Oxoglutarate	NULL		favours	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_2_16796668_s_8	16796668	2-Oxoglutarate favours complex formation  between PipX and NtcA, but impairs binding to PII, suggesting that partner  swapping between these nitrogen regulators is driven by the 2-oxoglutarate  concentration.	bind
27945	3	7249	7	NULL	NULL	0	NULL	2-Oxoglutarate	NULL		impairs	NULL				PII	NULL	binding to			NULL		0	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_2_16796668_s_8	16796668	2-Oxoglutarate favours complex formation  between PipX and NtcA, but impairs binding to PII, suggesting that partner  swapping between these nitrogen regulators is driven by the 2-oxoglutarate  concentration.	bind
27946	4	7249	7	NULL	NULL	0	NULL	2-Oxoglutarate	NULL		swaps	NULL				PipX	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_2_16796668_s_8	16796668	2-Oxoglutarate favours complex formation  between PipX and NtcA, but impairs binding to PII, suggesting that partner  swapping between these nitrogen regulators is driven by the 2-oxoglutarate  concentration.	bind
27947	5	7249	7	NULL	NULL	0	NULL	2-Oxoglutarate	NULL		swaps	NULL				NtcA	NULL				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_2_16796668_s_8	16796668	2-Oxoglutarate favours complex formation  between PipX and NtcA, but impairs binding to PII, suggesting that partner  swapping between these nitrogen regulators is driven by the 2-oxoglutarate  concentration.	bind
27948	6	7249	7	NULL	NULL	0	NULL	PipX	NULL		is a type of	NULL				nitrogen regulator	NULL				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_2_16796668_s_8	16796668	2-Oxoglutarate favours complex formation  between PipX and NtcA, but impairs binding to PII, suggesting that partner  swapping between these nitrogen regulators is driven by the 2-oxoglutarate  concentration.	bind
27949	7	7249	7	NULL	NULL	0	NULL	NtcA	NULL		is a type of	NULL				nitrogen regulator	NULL				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_2_16796668_s_8	16796668	2-Oxoglutarate favours complex formation  between PipX and NtcA, but impairs binding to PII, suggesting that partner  swapping between these nitrogen regulators is driven by the 2-oxoglutarate  concentration.	bind
22877	1	7250	6	13	NULL	NULL	NULL	q12	Chromosome		bind									CpG regions	NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_18_6913_s_22	16624877	2-q12 and SP1 binding to CpG regions appears to be important for basal transcription ( ).	bind
22878	2	7250	6	13	NULL	NULL	NULL	Sp1	GP		bind									CpG regions	NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_18_6913_s_22	16624877	2-q12 and SP1 binding to CpG regions appears to be important for basal transcription ( ).	bind
22879	3	7250	6	13	NULL	NULL	NULL	statement 1	Process		is important for					basal transcription	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_18_6913_s_22	16624877	2-q12 and SP1 binding to CpG regions appears to be important for basal transcription ( ).	bind
22880	4	7250	6	13	NULL	NULL	NULL	statement 2	Process		is important for					basal transcription	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_18_6913_s_22	16624877	2-q12 and SP1 binding to CpG regions appears to be important for basal transcription ( ).	bind
27950	1	7250	7	NULL	NULL	0	NULL	2-q12	NULL		bind	NULL					NULL			CpG region	NULL		0	NULL	NULL	NULL	gw70_pnas_103_18_6913_s_22	16624877	2-q12 and SP1 binding to CpG regions appears to be important for basal transcription ( ).	bind
27951	2	7250	7	NULL	NULL	0	NULL	SP1	NULL		bind	NULL					NULL			CpG region	NULL		0	NULL	NULL	NULL	gw70_pnas_103_18_6913_s_22	16624877	2-q12 and SP1 binding to CpG regions appears to be important for basal transcription ( ).	bind
27952	3	7250	7	NULL	NULL	0	NULL	statement 1	NULL		is important for	NULL				basal transcription	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_103_18_6913_s_22	16624877	2-q12 and SP1 binding to CpG regions appears to be important for basal transcription ( ).	bind
27953	4	7250	7	NULL	NULL	0	NULL	statement 2	NULL		is important for	NULL				basal transcription	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_103_18_6913_s_22	16624877	2-q12 and SP1 binding to CpG regions appears to be important for basal transcription ( ).	bind
22881	1	7252	6	13	NULL	NULL	NULL	salicylhydroxamic acid	Chemical		bind					myeloperoxidase	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_annurevbiophysbiomol_32_0_183_s_473	12574066	2.3  Ang  resolution X-ray crystal structure of the bisubstrate  analogue inhibitor salicylhydroxamic acid bound to human myeloperoxidase: a model  for a prereaction complex with hydroperoxide.	bind
46506	2	7252	6	13	NULL	NULL	NULL	salicylhydroxamic acid	Chemical		is a type of					bisubstrate analogue inhibitor	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiophysbiomol_32_0_183_s_473	12574066	2.3  Ang  resolution X-ray crystal structure of the bisubstrate  analogue inhibitor salicylhydroxamic acid bound to human myeloperoxidase: a model  for a prereaction complex with hydroperoxide.	bind
27954	1	7252	7	NULL	NULL	0	NULL	salicylhydroxamic acid	NULL		bind	NULL				 myeloperoxidase	NULL	human			NULL		0	NULL	NULL	NULL	gw70_annurevbiophysbiomol_32_0_183_s_473	12574066	2.3  Ang  resolution X-ray crystal structure of the bisubstrate  analogue inhibitor salicylhydroxamic acid bound to human myeloperoxidase: a model  for a prereaction complex with hydroperoxide.	bind
27955	2	7252	7	NULL	NULL	0	NULL	salicylhydroxamic acid	NULL		is a type of	NULL				bisubstrate analogue inhibitor 	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevbiophysbiomol_32_0_183_s_473	12574066	2.3  Ang  resolution X-ray crystal structure of the bisubstrate  analogue inhibitor salicylhydroxamic acid bound to human myeloperoxidase: a model  for a prereaction complex with hydroperoxide.	bind
22882	1	7253	6	13	NULL	NULL	NULL	flavosemiquinone	Chemical		is					FSQ	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_biochemistry_31_46_1445874_s_3	1445874	2.3)  are modified by the product pyruvate, which binds to the flavosemiquinone  (FSQ) form of the prosthetic flavin and decreases the thermodynamic driving  force for electron transfer from FSQ to heme.	bind
22883	2	7253	6	13	NULL	NULL	NULL	pyruvate	Chemical		bind					prosthetic flavin	Chemical	FSQ form of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_biochemistry_31_46_1445874_s_3	1445874	2.3)  are modified by the product pyruvate, which binds to the flavosemiquinone  (FSQ) form of the prosthetic flavin and decreases the thermodynamic driving  force for electron transfer from FSQ to heme.	bind
22956	3	7253	6	13	NULL	NULL	NULL	electron	Chemical		transfered to					heme	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_biochemistry_31_46_1445874_s_3	1445874	2.3)  are modified by the product pyruvate, which binds to the flavosemiquinone  (FSQ) form of the prosthetic flavin and decreases the thermodynamic driving  force for electron transfer from FSQ to heme.	bind
22957	4	7253	6	13	NULL	NULL	NULL	pyruvate	Chemical		decreases					statement 7	Process	thermodynamic driving force of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_biochemistry_31_46_1445874_s_3	1445874	2.3)  are modified by the product pyruvate, which binds to the flavosemiquinone  (FSQ) form of the prosthetic flavin and decreases the thermodynamic driving  force for electron transfer from FSQ to heme.	bind
53637	6	7253	6	13	NULL	NULL	NULL	electron	Chemical		is transfered from					FSQ	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_biochemistry_31_46_1445874_s_3	1445874	2.3)  are modified by the product pyruvate, which binds to the flavosemiquinone  (FSQ) form of the prosthetic flavin and decreases the thermodynamic driving  force for electron transfer from FSQ to heme.	bind
53638	7	7253	6	13	NULL	NULL	NULL	statement 3	Process		occurs simultaneously with					statement 6	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_biochemistry_31_46_1445874_s_3	1445874	2.3)  are modified by the product pyruvate, which binds to the flavosemiquinone  (FSQ) form of the prosthetic flavin and decreases the thermodynamic driving  force for electron transfer from FSQ to heme.	bind
27956	1	7253	7	NULL	NULL	0	NULL	pyruvate	NULL		binds to	NULL				prosthetic flavin	NULL	FSQ form of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_biochemistry_31_46_1445874_s_3	1445874	2.3)  are modified by the product pyruvate, which binds to the flavosemiquinone  (FSQ) form of the prosthetic flavin and decreases the thermodynamic driving  force for electron transfer from FSQ to heme.	bind
27957	2	7253	7	10	NULL	0	NULL	electron	NULL		is transfered from	NULL				FSQ	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_biochemistry_31_46_1445874_s_3	1445874	2.3)  are modified by the product pyruvate, which binds to the flavosemiquinone  (FSQ) form of the prosthetic flavin and decreases the thermodynamic driving  force for electron transfer from FSQ to heme.	bind
27958	3	7253	7	10	NULL	0	NULL	pyruvate	NULL		decrease	NULL				statement 6	NULL	thermodynamic driving force of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_biochemistry_31_46_1445874_s_3	1445874	2.3)  are modified by the product pyruvate, which binds to the flavosemiquinone  (FSQ) form of the prosthetic flavin and decreases the thermodynamic driving  force for electron transfer from FSQ to heme.	bind
53636	4	7253	7	10	NULL	0	NULL	FSQ	NULL		is	NULL				flavosemiquinone	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochemistry_31_46_1445874_s_3	1445874	2.3)  are modified by the product pyruvate, which binds to the flavosemiquinone  (FSQ) form of the prosthetic flavin and decreases the thermodynamic driving  force for electron transfer from FSQ to heme.	bind
53639	5	7253	7	10	NULL	0	NULL	electron	NULL		is transfered to	NULL				heme	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochemistry_31_46_1445874_s_3	1445874	2.3)  are modified by the product pyruvate, which binds to the flavosemiquinone  (FSQ) form of the prosthetic flavin and decreases the thermodynamic driving  force for electron transfer from FSQ to heme.	bind
53640	6	7253	7	10	NULL	0	NULL	statement 2	NULL		occurs simultaneously with	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochemistry_31_46_1445874_s_3	1445874	2.3)  are modified by the product pyruvate, which binds to the flavosemiquinone  (FSQ) form of the prosthetic flavin and decreases the thermodynamic driving  force for electron transfer from FSQ to heme.	bind
22884	1	7255	6	13	NULL	NULL	NULL	Ase1p	GP		bind					MT	CellComponent	taxol-stabilized			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_160_4_517_s_115	12591913	2.5 mug of (BV)Ase1p was bound to Taxol-stabilized  MTs as in  Fig. 3 A (s, supernatant; p, pellet).	bind
27959	1	7255	7	NULL	NULL	0	NULL	Ase1p	NULL		bind	NULL				MTs	NULL	 Taxol-stabilized 			NULL		0	NULL	NULL	NULL	gw70_cellbiol_160_4_517_s_115	12591913	2.5 mug of (BV)Ase1p was bound to Taxol-stabilized  MTs as in  Fig. 3 A (s, supernatant; p, pellet).	bind
22885	1	7258	6	13	NULL	NULL	NULL	Sp1 	GP		bind					DNA	NucleicAcid			GC box	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_4920_s_294	11812820	20       Kuwahara,J., Yonezawa,A., Futamura,M. and Sugiura,Y. (1993) Binding of transcription factor Sp1 to GC box DNA revealed by footprinting analysis: different contact of three zinc fingers and sequence recognition mode.	bind
46507	2	7258	6	13	NULL	NULL	NULL	Sp1	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_4920_s_294	11812820	20       Kuwahara,J., Yonezawa,A., Futamura,M. and Sugiura,Y. (1993) Binding of transcription factor Sp1 to GC box DNA revealed by footprinting analysis: different contact of three zinc fingers and sequence recognition mode.	bind
27960	1	7258	7	10	NULL	0	NULL	 Sp1	NULL		bind	NULL				DNA	NULL			GC box	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_4920_s_294	11812820	20       Kuwahara,J., Yonezawa,A., Futamura,M. and Sugiura,Y. (1993) Binding of transcription factor Sp1 to GC box DNA revealed by footprinting analysis: different contact of three zinc fingers and sequence recognition mode.	bind
46509	2	7258	7	10	NULL	0	NULL	Sp1	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_4920_s_294	11812820	20       Kuwahara,J., Yonezawa,A., Futamura,M. and Sugiura,Y. (1993) Binding of transcription factor Sp1 to GC box DNA revealed by footprinting analysis: different contact of three zinc fingers and sequence recognition mode.	bind
22886	1	7259	6	13	NULL	NULL	NULL	Mot3	GP		bind					Ty	NucleicAcid	Saccharomyces cerevisiae		long terminal repeat (delta)	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_799_s_357	11160904	20       Madison,J.M., Dudley,A.M. and Winston,F. (1998) Identification and analysis of Mot3, a zinc finger protein that binds to the retrotransposon Ty long terminal repeat (delta) in  Saccharomyces cerevisiae.	bind
46510	2	7259	6	13	NULL	NULL	NULL	Mot3	GP		is a type of					zinc finger protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_799_s_357	11160904	20       Madison,J.M., Dudley,A.M. and Winston,F. (1998) Identification and analysis of Mot3, a zinc finger protein that binds to the retrotransposon Ty long terminal repeat (delta) in  Saccharomyces cerevisiae.	bind
46511	3	7259	6	13	NULL	NULL	NULL	Ty	NucleicAcid		is a type of					retrotransposon	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_799_s_357	11160904	20       Madison,J.M., Dudley,A.M. and Winston,F. (1998) Identification and analysis of Mot3, a zinc finger protein that binds to the retrotransposon Ty long terminal repeat (delta) in  Saccharomyces cerevisiae.	bind
27961	1	7259	7	10	NULL	0	NULL	Mot3	NULL		binds to	NULL				Ty	NULL	Saccharomyces cerevisiae		long terminal repeat (delta)	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_799_s_357	11160904	20       Madison,J.M., Dudley,A.M. and Winston,F. (1998) Identification and analysis of Mot3, a zinc finger protein that binds to the retrotransposon Ty long terminal repeat (delta) in  Saccharomyces cerevisiae.	bind
27962	2	7259	7	NULL	NULL	0	NULL	Mot3	NULL		is a type of	NULL				zinc finger protein	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_799_s_357	11160904	20       Madison,J.M., Dudley,A.M. and Winston,F. (1998) Identification and analysis of Mot3, a zinc finger protein that binds to the retrotransposon Ty long terminal repeat (delta) in  Saccharomyces cerevisiae.	bind
27963	3	7259	7	10	NULL	0	NULL	Ty	NULL		is a type of	NULL				retrotransposon	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_799_s_357	11160904	20       Madison,J.M., Dudley,A.M. and Winston,F. (1998) Identification and analysis of Mot3, a zinc finger protein that binds to the retrotransposon Ty long terminal repeat (delta) in  Saccharomyces cerevisiae.	bind
22887	1	7260	6	13	NULL	NULL	NULL	L5	GP	Xenopus laevis	bind					5S rRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2510_s_288	11410658	20       Wormington,W.M. (1989) Developmental expression and 5S rRNA-binding activity of  Xenopus laevis ribosomal protein L5.	bind
46512	2	7260	6	13	NULL	NULL	NULL	L5	GP		is a type of					ribosomal protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2510_s_288	11410658	20       Wormington,W.M. (1989) Developmental expression and 5S rRNA-binding activity of  Xenopus laevis ribosomal protein L5.	bind
27964	1	7260	7	NULL	NULL	0	NULL	5S rRNA	NULL		bind	NULL				L5	NULL	Xenopus laevis			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2510_s_288	11410658	20       Wormington,W.M. (1989) Developmental expression and 5S rRNA-binding activity of  Xenopus laevis ribosomal protein L5.	bind
27965	2	7260	7	NULL	NULL	0	NULL	L5	NULL		is a type of	NULL				ribosomal protein	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2510_s_288	11410658	20       Wormington,W.M. (1989) Developmental expression and 5S rRNA-binding activity of  Xenopus laevis ribosomal protein L5.	bind
22888	1	7261	6	13	NULL	NULL	NULL	factor VIIa	GP		bind					tissue factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_21_2555_s_125	11382723	20  23  This mechanism may also explain why the plasma level of recombinant factor VIIa required for adequate hemostatic efficiency far exceeds the  Kd for binding of factor VIIa to tissue factor.	bind
22889	2	7261	6	13	NULL	NULL	NULL	factor VIIa	GP	recombinant	required for					hemostatic efficiency	Process	adequate 			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_21_2555_s_125	11382723	20  23  This mechanism may also explain why the plasma level of recombinant factor VIIa required for adequate hemostatic efficiency far exceeds the  Kd for binding of factor VIIa to tissue factor.	bind
27966	1	7261	7	10	NULL	0	NULL	factor VIIa	NULL		bind	NULL				tissue factor	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_21_2555_s_125	11382723	20  23  This mechanism may also explain why the plasma level of recombinant factor VIIa required for adequate hemostatic efficiency far exceeds the  Kd for binding of factor VIIa to tissue factor.	bind
27967	2	7261	7	10	NULL	0	NULL	factor VIIa	NULL	recombinant	is required for	NULL				hemostatic efficiency	NULL	adequate			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_21_2555_s_125	11382723	20  23  This mechanism may also explain why the plasma level of recombinant factor VIIa required for adequate hemostatic efficiency far exceeds the  Kd for binding of factor VIIa to tissue factor.	bind
22890	1	7262	6	13	NULL	NULL	NULL	TGF-alpha	GP		bind					EGF-R	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_4_1307_s_158	10751356	20  Following inhalation of asbestos by rats, transforming growth factor-alpha (TGF-alpha), which can bind EGF-R, is also up-regulated with corresponding increases in cellular proliferation within developing asbestotic lesions.	bind
22891	2	7262	6	13	NULL	NULL	NULL	TGF-alpha	GP		is					transforming growth factor-alpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_4_1307_s_158	10751356	20  Following inhalation of asbestos by rats, transforming growth factor-alpha (TGF-alpha), which can bind EGF-R, is also up-regulated with corresponding increases in cellular proliferation within developing asbestotic lesions.	bind
22892	3	7262	6	13	NULL	NULL	NULL	TGF-alpha	GP		is upregulated with					cellular proliferation	Process	increase in			NULL	developing asbestotic lesions	NULL	NULL	NULL	NULL	gw60_amjpathol_156_4_1307_s_158	10751356	20  Following inhalation of asbestos by rats, transforming growth factor-alpha (TGF-alpha), which can bind EGF-R, is also up-regulated with corresponding increases in cellular proliferation within developing asbestotic lesions.	bind
53643	4	7262	6	13	NULL	NULL	NULL	asbestos	Chemical		upregulates					TGF-alpha	GP				NULL	rats	NULL	NULL	NULL	NULL	gw60_amjpathol_156_4_1307_s_158	10751356	20  Following inhalation of asbestos by rats, transforming growth factor-alpha (TGF-alpha), which can bind EGF-R, is also up-regulated with corresponding increases in cellular proliferation within developing asbestotic lesions.	bind
27968	1	7262	7	NULL	NULL	0	NULL	TGF-alpha	NULL		bind	NULL				EGF-R	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_4_1307_s_158	10751356	20  Following inhalation of asbestos by rats, transforming growth factor-alpha (TGF-alpha), which can bind EGF-R, is also up-regulated with corresponding increases in cellular proliferation within developing asbestotic lesions.	bind
27969	2	7262	7	10	NULL	0	NULL	asbestos	NULL		upregulates	NULL				TGF-alpha	NULL				NULL	rats	NULL	NULL	NULL	NULL	gw60_amjpathol_156_4_1307_s_158	10751356	20  Following inhalation of asbestos by rats, transforming growth factor-alpha (TGF-alpha), which can bind EGF-R, is also up-regulated with corresponding increases in cellular proliferation within developing asbestotic lesions.	bind
27970	3	7262	7	10	NULL	0	NULL	TGF-alpha	NULL		is upregulated with	NULL				cellular proliferation	NULL	increase in			NULL	developing asbestotic lesions	NULL	NULL	NULL	NULL	gw60_amjpathol_156_4_1307_s_158	10751356	20  Following inhalation of asbestos by rats, transforming growth factor-alpha (TGF-alpha), which can bind EGF-R, is also up-regulated with corresponding increases in cellular proliferation within developing asbestotic lesions.	bind
27971	4	7262	7	NULL	NULL	0	NULL	TGF-alpha	NULL		is	NULL				transforming growth factor-alpha	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_4_1307_s_158	10751356	20  Following inhalation of asbestos by rats, transforming growth factor-alpha (TGF-alpha), which can bind EGF-R, is also up-regulated with corresponding increases in cellular proliferation within developing asbestotic lesions.	bind
22893	1	7263	6	13	NULL	NULL	NULL	EC-SOD	GP	subtype of	is bound to					endothelium	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_19_2264_s_152	10811593	20  Heparin specifically binds the subtype of EC-SOD (type C) that is bound to the endothelium.	bind
22894	2	7263	6	13	NULL	NULL	NULL	heparin	Chemical		bind		specifically			statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_19_2264_s_152	10811593	20  Heparin specifically binds the subtype of EC-SOD (type C) that is bound to the endothelium.	bind
27972	1	7263	7	NULL	NULL	0	NULL	EC-SOD	NULL	subtype of	bind	NULL				 endothelium	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_19_2264_s_152	10811593	20  Heparin specifically binds the subtype of EC-SOD (type C) that is bound to the endothelium.	bind
27973	2	7263	7	NULL	NULL	0	NULL	Heparin 	NULL		binds	NULL	specifically			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_19_2264_s_152	10811593	20  Heparin specifically binds the subtype of EC-SOD (type C) that is bound to the endothelium.	bind
22895	1	7264	6	13	NULL	NULL	NULL	polyclonal anti - c-Src antibody	GP	rabbit	bind					protein A	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_8_672_s_75	10521240	20  Immunoprecipitates prepared with rabbit polyclonal anti - c-Src antibody bound to protein A - Sepharose beads were incubated for 10 minutes at 30 degrees C with an assay buffer containing (in mmol/L) Tris-HCl (pH 7.2) 100, MgCl2 125, MnCl2 25, EGTA 2, Na2VO4 0.25, and DTT 2, and 125 mumol/L cold ATP and 10 muCi of [gamma-32]ATP.	bind
27974	1	7264	7	NULL	NULL	0	NULL	  polyclonal anti - c-Src antibody	NULL	rabbit	bind	NULL				protein A	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_8_672_s_75	10521240	20  Immunoprecipitates prepared with rabbit polyclonal anti - c-Src antibody bound to protein A - Sepharose beads were incubated for 10 minutes at 30 degrees C with an assay buffer containing (in mmol/L) Tris-HCl (pH 7.2) 100, MgCl2 125, MnCl2 25, EGTA 2, Na2VO4 0.25, and DTT 2, and 125 mumol/L cold ATP and 10 muCi of [gamma-32]ATP.	bind
22896	1	7265	6	13	NULL	NULL	NULL	alpha2beta1 integrin	GP		bind					collagen	GP	native			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_5_1489_s_92	10793060	20  In addition, the alpha2beta1 integrin which binds native collagen showed minimal binding to denatured collagen.	bind
22897	2	7265	6	13	NULL	NULL	NULL	alpha2beta1 integrin	GP		bind		minimally			collagen	GP	denatured			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_5_1489_s_92	10793060	20  In addition, the alpha2beta1 integrin which binds native collagen showed minimal binding to denatured collagen.	bind
27975	1	7265	7	NULL	NULL	0	NULL	alpha2beta1 integrin	NULL		binds	NULL				collagen	NULL	native			NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_5_1489_s_92	10793060	20  In addition, the alpha2beta1 integrin which binds native collagen showed minimal binding to denatured collagen.	bind
27976	2	7265	7	NULL	NULL	0	NULL	alpha2beta1 integrin	NULL		binds	NULL	minimally			collagen	NULL	denatured			NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_5_1489_s_92	10793060	20  In addition, the alpha2beta1 integrin which binds native collagen showed minimal binding to denatured collagen.	bind
22898	1	7266	6	13	NULL	NULL	NULL	Rnd1	GP		bind		constitutively			GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_3_173_s_50	10926864	20  Rnd1 is constitutively bound to GTP and able to block Ca2+ sensitization by RhoA.	bind
22899	2	7266	6	13	NULL	NULL	NULL	RhoA	GP		plays a role in					Ca2+	Chemical	sensitization of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_3_173_s_50	10926864	20  Rnd1 is constitutively bound to GTP and able to block Ca2+ sensitization by RhoA.	bind
22900	3	7266	6	13	NULL	NULL	NULL	Rnd1	GP		block					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_3_173_s_50	10926864	20  Rnd1 is constitutively bound to GTP and able to block Ca2+ sensitization by RhoA.	bind
27977	1	7266	7	NULL	NULL	0	NULL	Rnd1 	NULL		binds	NULL	constitutively			GTP	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_3_173_s_50	10926864	20  Rnd1 is constitutively bound to GTP and able to block Ca2+ sensitization by RhoA.	bind
27978	2	7266	7	NULL	NULL	0	NULL	RhoA	NULL		sensitize	NULL				Ca2+	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_3_173_s_50	10926864	20  Rnd1 is constitutively bound to GTP and able to block Ca2+ sensitization by RhoA.	bind
27979	3	7266	7	NULL	NULL	0	NULL	statement 1	NULL		block	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_3_173_s_50	10926864	20  Rnd1 is constitutively bound to GTP and able to block Ca2+ sensitization by RhoA.	bind
22901	1	7267	6	13	NULL	NULL	NULL	hypoxia	MedicalFinding		increases					Egr-1	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2029_s_87	10479642	20  Studies are in progress to trace the sequence of events increasing Egr-1 activation in hypoxia, and preliminary results indicate that oxygen deprivation enhances de novo Egr-1 synthesis and that this is driven by binding of ternary complex factor to ets/SRE sites in the Egr-1 promoter.	bind
22902	2	7267	6	13	NULL	NULL	NULL	oxygen 	Chemical	deprivation of	enhances					Egr-1	GP	de novo synthesis of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2029_s_87	10479642	20  Studies are in progress to trace the sequence of events increasing Egr-1 activation in hypoxia, and preliminary results indicate that oxygen deprivation enhances de novo Egr-1 synthesis and that this is driven by binding of ternary complex factor to ets/SRE sites in the Egr-1 promoter.	bind
22903	3	7267	6	13	NULL	NULL	NULL	ternary complex factor	GP		bind					Egr-1 	GP			ets/SRE sites of the promoter	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2029_s_87	10479642	20  Studies are in progress to trace the sequence of events increasing Egr-1 activation in hypoxia, and preliminary results indicate that oxygen deprivation enhances de novo Egr-1 synthesis and that this is driven by binding of ternary complex factor to ets/SRE sites in the Egr-1 promoter.	bind
27980	1	7267	7	NULL	NULL	0	NULL	oxygen	NULL	deprivation of	enhance	NULL				Egr-1	NULL	de novo synthesis of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2029_s_87	10479642	20  Studies are in progress to trace the sequence of events increasing Egr-1 activation in hypoxia, and preliminary results indicate that oxygen deprivation enhances de novo Egr-1 synthesis and that this is driven by binding of ternary complex factor to ets/SRE sites in the Egr-1 promoter.	bind
27981	2	7267	7	NULL	NULL	0	NULL	ternary complex factor 	NULL		bind	NULL				 Egr-1	NULL			ets/SRE sites in the promoter	NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2029_s_87	10479642	20  Studies are in progress to trace the sequence of events increasing Egr-1 activation in hypoxia, and preliminary results indicate that oxygen deprivation enhances de novo Egr-1 synthesis and that this is driven by binding of ternary complex factor to ets/SRE sites in the Egr-1 promoter.	bind
27982	3	7267	7	NULL	NULL	0	NULL	statement 2	NULL		drives	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2029_s_87	10479642	20  Studies are in progress to trace the sequence of events increasing Egr-1 activation in hypoxia, and preliminary results indicate that oxygen deprivation enhances de novo Egr-1 synthesis and that this is driven by binding of ternary complex factor to ets/SRE sites in the Egr-1 promoter.	bind
22904	1	7268	6	13	NULL	NULL	NULL	FXa	GP		bind					TF	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_5_1362_s_34	10807755	20  TFPI uses the tandem Kunitz-type domains in its structure to form a quaternary complex with FXa bound to TF .	bind
22905	2	7268	6	13	NULL	NULL	NULL	TFPI	GP		form a quaternary complex with			tandem Kunitz-type domains		statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_5_1362_s_34	10807755	20  TFPI uses the tandem Kunitz-type domains in its structure to form a quaternary complex with FXa bound to TF .	bind
27983	1	7268	7	NULL	NULL	0	NULL	FXa 	NULL		bind	NULL				TF	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_5_1362_s_34	10807755	20  TFPI uses the tandem Kunitz-type domains in its structure to form a quaternary complex with FXa bound to TF .	bind
27984	2	7268	7	NULL	NULL	0	NULL	TFPI	NULL		form quaternary complex with	NULL		tandem Kunitz-type domain		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_5_1362_s_34	10807755	20  TFPI uses the tandem Kunitz-type domains in its structure to form a quaternary complex with FXa bound to TF .	bind
22906	1	7269	6	13	NULL	NULL	NULL	fibrinogen	GP		bind					glycoprotein IIb/IIa complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3461_s_36	9437193	20 21  Binding of fibrinogen to the glycoprotein IIb/IIa complex appears to be the final common pathway for platelet aggregation.	bind
22907	2	7269	6	13	NULL	NULL	NULL	statement 1	Process		is needed for					platelet aggregation	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3461_s_36	9437193	20 21  Binding of fibrinogen to the glycoprotein IIb/IIa complex appears to be the final common pathway for platelet aggregation.	bind
27985	1	7269	7	NULL	NULL	0	NULL	fibrinogen	NULL		bind	NULL				glycoprotein IIb/IIa complex	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3461_s_36	9437193	20 21  Binding of fibrinogen to the glycoprotein IIb/IIa complex appears to be the final common pathway for platelet aggregation.	bind
27986	2	7269	7	NULL	NULL	0	NULL	statement 1	NULL		is the pathway for	NULL				platelet aggregation	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3461_s_36	9437193	20 21  Binding of fibrinogen to the glycoprotein IIb/IIa complex appears to be the final common pathway for platelet aggregation.	bind
22908	1	7270	6	13	NULL	NULL	NULL	heparin	Chemical		bind					thrombin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_10_1158_s_189	10715263	20 21  Heparin binds to various other partners besides thrombin and is thereby inhibited.	bind
27987	1	7270	7	NULL	NULL	0	NULL	Heparin	NULL		binds to	NULL				thrombin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_101_10_1158_s_189	10715263	20 21  Heparin binds to various other partners besides thrombin and is thereby inhibited.	bind
27988	2	7270	7	NULL	NULL	0	NULL	statement 1	NULL		inhibits	NULL				thrombin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_101_10_1158_s_189	10715263	20 21  Heparin binds to various other partners besides thrombin and is thereby inhibited.	bind
22909	1	7271	6	13	NULL	NULL	NULL	heparin/HS	Chemical		bind					bFGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_7_1853_s_22	9107173	20 21 22  Polyaromatic heparin-mimicking anionic molecules compete with heparin/HS for bFGF binding and hence inhibit bFGF receptor binding and mitogenic activity.	bind
22910	2	7271	6	13	NULL	NULL	NULL	Polyaromatic heparin-mimicking anionic molecules	Chemical		bind					bFGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_7_1853_s_22	9107173	20 21 22  Polyaromatic heparin-mimicking anionic molecules compete with heparin/HS for bFGF binding and hence inhibit bFGF receptor binding and mitogenic activity.	bind
22911	3	7271	6	13	NULL	NULL	NULL	statement 1	Process		competes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_7_1853_s_22	9107173	20 21 22  Polyaromatic heparin-mimicking anionic molecules compete with heparin/HS for bFGF binding and hence inhibit bFGF receptor binding and mitogenic activity.	bind
22913	5	7271	6	13	NULL	NULL	NULL	statement 3	Process		inhibits					bFGF receptor	GP	mitogenic activity of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_7_1853_s_22	9107173	20 21 22  Polyaromatic heparin-mimicking anionic molecules compete with heparin/HS for bFGF binding and hence inhibit bFGF receptor binding and mitogenic activity.	bind
22914	6	7271	6	13	NULL	NULL	NULL	statement 3	Process		inhibits					bFGF receptor	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_7_1853_s_22	9107173	20 21 22  Polyaromatic heparin-mimicking anionic molecules compete with heparin/HS for bFGF binding and hence inhibit bFGF receptor binding and mitogenic activity.	bind
27989	1	7271	7	NULL	NULL	0	NULL	heparin/HS	NULL		bind	NULL				bFGF	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_95_7_1853_s_22	9107173	20 21 22  Polyaromatic heparin-mimicking anionic molecules compete with heparin/HS for bFGF binding and hence inhibit bFGF receptor binding and mitogenic activity.	bind
27990	2	7271	7	NULL	NULL	0	NULL	Polyaromatic heparin-mimicking anionic molecules	NULL		bind	NULL				bFGF	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_95_7_1853_s_22	9107173	20 21 22  Polyaromatic heparin-mimicking anionic molecules compete with heparin/HS for bFGF binding and hence inhibit bFGF receptor binding and mitogenic activity.	bind
27991	3	7271	7	NULL	NULL	0	NULL	statement 1	NULL		compete with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_95_7_1853_s_22	9107173	20 21 22  Polyaromatic heparin-mimicking anionic molecules compete with heparin/HS for bFGF binding and hence inhibit bFGF receptor binding and mitogenic activity.	bind
27992	4	7271	7	NULL	NULL	0	NULL	statement 2	NULL		inhibit	NULL				bFGF receptor	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_circulation_95_7_1853_s_22	9107173	20 21 22  Polyaromatic heparin-mimicking anionic molecules compete with heparin/HS for bFGF binding and hence inhibit bFGF receptor binding and mitogenic activity.	bind
27993	5	7271	7	NULL	NULL	0	NULL	statement 2	NULL		inhibit	NULL				bFGF receptor	NULL	mitogenic activity of			NULL		0	NULL	NULL	NULL	gw60_circulation_95_7_1853_s_22	9107173	20 21 22  Polyaromatic heparin-mimicking anionic molecules compete with heparin/HS for bFGF binding and hence inhibit bFGF receptor binding and mitogenic activity.	bind
22959	1	7272	6	13	NULL	NULL	NULL	tryp-VLDL	GP		bind		high affinity;;specificity			macrophage receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_968_s_200	9633939	20 21 22  The tryp-VLDL bound with high affinity and specificity to this macrophage receptor and MBP 200, 235 and failed to bind to the LDL receptor.	bind
22960	2	7272	6	13	NULL	NULL	NULL	tryp-VLDL	GP		bind		high affinity;;specificity			MBP 200	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_968_s_200	9633939	20 21 22  The tryp-VLDL bound with high affinity and specificity to this macrophage receptor and MBP 200, 235 and failed to bind to the LDL receptor.	bind
22961	3	7272	6	13	NULL	NULL	NULL	tryp-VLDL	GP		bind		high affinity;;specificity			MBP 235	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_968_s_200	9633939	20 21 22  The tryp-VLDL bound with high affinity and specificity to this macrophage receptor and MBP 200, 235 and failed to bind to the LDL receptor.	bind
22962	4	7272	6	13	NULL	NULL	NULL	tryp-VLDL	GP		does not bind					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_968_s_200	9633939	20 21 22  The tryp-VLDL bound with high affinity and specificity to this macrophage receptor and MBP 200, 235 and failed to bind to the LDL receptor.	bind
27994	1	7272	7	NULL	NULL	0	NULL	tryp-VLDL	NULL		bind	NULL	high affinity;;specificity			macrophage receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_968_s_200	9633939	20 21 22  The tryp-VLDL bound with high affinity and specificity to this macrophage receptor and MBP 200, 235 and failed to bind to the LDL receptor.	bind
27995	2	7272	7	NULL	NULL	0	NULL	tryp-VLDL	NULL		bind	NULL	high affinity;;specificity			MBP 200	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_968_s_200	9633939	20 21 22  The tryp-VLDL bound with high affinity and specificity to this macrophage receptor and MBP 200, 235 and failed to bind to the LDL receptor.	bind
27996	3	7272	7	NULL	NULL	0	NULL	tryp-VLDL	NULL		bind	NULL	high affinity;;specificity			MBP 235	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_968_s_200	9633939	20 21 22  The tryp-VLDL bound with high affinity and specificity to this macrophage receptor and MBP 200, 235 and failed to bind to the LDL receptor.	bind
27997	4	7272	7	NULL	NULL	0	NULL	tryp-VLDL	NULL		does not bind	NULL				LDL receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_968_s_200	9633939	20 21 22  The tryp-VLDL bound with high affinity and specificity to this macrophage receptor and MBP 200, 235 and failed to bind to the LDL receptor.	bind
22963	1	7273	6	13	NULL	NULL	NULL	ets proteins	GP		bind					GGA core	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_585_s_159	10669659	20 21 32  The  ets proteins are members of a large family with a conserved 84 - amino acid sequence (the  ets domain) allowing their binding to the GGA core as monomers.	bind
22964	2	7273	6	13	NULL	NULL	NULL	ets protein members	GP		have conserved 								ETS domain		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_585_s_159	10669659	20 21 32  The  ets proteins are members of a large family with a conserved 84 - amino acid sequence (the  ets domain) allowing their binding to the GGA core as monomers.	bind
46518	3	7273	6	13	NULL	NULL	NULL	GGA core	NucleicAcid		occur as					monomers	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_585_s_159	10669659	20 21 32  The  ets proteins are members of a large family with a conserved 84 - amino acid sequence (the  ets domain) allowing their binding to the GGA core as monomers.	bind
27998	1	7273	7	NULL	NULL	0	NULL	ets protein	NULL		bind	NULL				GGA core	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_585_s_159	10669659	20 21 32  The  ets proteins are members of a large family with a conserved 84 - amino acid sequence (the  ets domain) allowing their binding to the GGA core as monomers.	bind
27999	2	7273	7	NULL	NULL	0	NULL	ets protein	NULL		are members of	NULL					NULL		ets domain family		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_585_s_159	10669659	20 21 32  The  ets proteins are members of a large family with a conserved 84 - amino acid sequence (the  ets domain) allowing their binding to the GGA core as monomers.	bind
28000	3	7273	7	NULL	NULL	0	NULL	ets domain	NULL		contains	NULL					NULL		conserved 84 - amino acid sequence		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_585_s_159	10669659	20 21 32  The  ets proteins are members of a large family with a conserved 84 - amino acid sequence (the  ets domain) allowing their binding to the GGA core as monomers.	bind
28001	4	7273	7	NULL	NULL	0	NULL	statement 1	NULL		occur as	NULL				monomers	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_585_s_159	10669659	20 21 32  The  ets proteins are members of a large family with a conserved 84 - amino acid sequence (the  ets domain) allowing their binding to the GGA core as monomers.	bind
22965	1	7274	6	13	NULL	NULL	NULL	Sp1	GP		bind									repeat 3	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_7_1777_s_221	10894816	20 35  A further difference between OM and IL-6 is that only IL-6 directly enhances the binding of Sp1 and Sp3 to repeat 3, whereas OM does not directly upregulate Sp1 binding activity.	bind
22966	2	7274	6	13	NULL	NULL	NULL	Sp3	GP		bind									repeat 3	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_7_1777_s_221	10894816	20 35  A further difference between OM and IL-6 is that only IL-6 directly enhances the binding of Sp1 and Sp3 to repeat 3, whereas OM does not directly upregulate Sp1 binding activity.	bind
22967	3	7274	6	13	NULL	NULL	NULL	IL-6	GP		enhances		directly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_7_1777_s_221	10894816	20 35  A further difference between OM and IL-6 is that only IL-6 directly enhances the binding of Sp1 and Sp3 to repeat 3, whereas OM does not directly upregulate Sp1 binding activity.	bind
22968	4	7274	6	13	NULL	NULL	NULL	IL-6	GP		enhances		directly			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_7_1777_s_221	10894816	20 35  A further difference between OM and IL-6 is that only IL-6 directly enhances the binding of Sp1 and Sp3 to repeat 3, whereas OM does not directly upregulate Sp1 binding activity.	bind
22969	5	7274	6	13	NULL	NULL	NULL	OM	GP		does not upregulate		directly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_7_1777_s_221	10894816	20 35  A further difference between OM and IL-6 is that only IL-6 directly enhances the binding of Sp1 and Sp3 to repeat 3, whereas OM does not directly upregulate Sp1 binding activity.	bind
28002	1	7274	7	10	NULL	0	NULL	Sp1			bind									repeat 3	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_7_1777_s_221	10894816	20 35  A further difference between OM and IL-6 is that only IL-6 directly enhances the binding of Sp1 and Sp3 to repeat 3, whereas OM does not directly upregulate Sp1 binding activity.	bind
28003	2	7274	7	10	NULL	0	NULL	Sp3			bind									repeat 3	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_7_1777_s_221	10894816	20 35  A further difference between OM and IL-6 is that only IL-6 directly enhances the binding of Sp1 and Sp3 to repeat 3, whereas OM does not directly upregulate Sp1 binding activity.	bind
28004	3	7274	7	NULL	NULL	0	NULL	 IL-6	NULL		enhance	NULL	directly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_7_1777_s_221	10894816	20 35  A further difference between OM and IL-6 is that only IL-6 directly enhances the binding of Sp1 and Sp3 to repeat 3, whereas OM does not directly upregulate Sp1 binding activity.	bind
28005	4	7274	7	NULL	NULL	0	NULL	IL-6	NULL		enhance	NULL	directly			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_7_1777_s_221	10894816	20 35  A further difference between OM and IL-6 is that only IL-6 directly enhances the binding of Sp1 and Sp3 to repeat 3, whereas OM does not directly upregulate Sp1 binding activity.	bind
28006	5	7274	7	NULL	NULL	0	NULL	OM	NULL		does not upregulate	NULL	directly			Sp1	NULL	binding activity of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_7_1777_s_221	10894816	20 35  A further difference between OM and IL-6 is that only IL-6 directly enhances the binding of Sp1 and Sp3 to repeat 3, whereas OM does not directly upregulate Sp1 binding activity.	bind
22970	1	7275	6	13	NULL	NULL	NULL	endothelin-1	GP		is					ET-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_3_221_s_37	12855672	20 Adrenergic agonists, endothelin-1 (ET-1), and angiotensin II (Ang II) binding to GPCR induce a rather uniform increase in cardiomyocyte size, resulting from the addition of myofibrils in parallel.	bind
22971	2	7275	6	13	NULL	NULL	NULL	angiotensin II	GP		is					Ang II	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_3_221_s_37	12855672	20 Adrenergic agonists, endothelin-1 (ET-1), and angiotensin II (Ang II) binding to GPCR induce a rather uniform increase in cardiomyocyte size, resulting from the addition of myofibrils in parallel.	bind
22972	3	7275	6	13	NULL	NULL	NULL	ET-1	GP		bind					GPCR	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_3_221_s_37	12855672	20 Adrenergic agonists, endothelin-1 (ET-1), and angiotensin II (Ang II) binding to GPCR induce a rather uniform increase in cardiomyocyte size, resulting from the addition of myofibrils in parallel.	bind
22973	4	7275	6	13	NULL	NULL	NULL	Ang II	GP		bind					GPCR	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_3_221_s_37	12855672	20 Adrenergic agonists, endothelin-1 (ET-1), and angiotensin II (Ang II) binding to GPCR induce a rather uniform increase in cardiomyocyte size, resulting from the addition of myofibrils in parallel.	bind
22974	5	7275	6	13	NULL	NULL	NULL	statement 3	Process		induce					cardiomyocyte size	Cell	increase in			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_3_221_s_37	12855672	20 Adrenergic agonists, endothelin-1 (ET-1), and angiotensin II (Ang II) binding to GPCR induce a rather uniform increase in cardiomyocyte size, resulting from the addition of myofibrils in parallel.	bind
22975	6	7275	6	13	NULL	NULL	NULL	statement 4	Process		induce					cardiomyocyte size	Cell	increase in			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_3_221_s_37	12855672	20 Adrenergic agonists, endothelin-1 (ET-1), and angiotensin II (Ang II) binding to GPCR induce a rather uniform increase in cardiomyocyte size, resulting from the addition of myofibrils in parallel.	bind
22976	7	7275	6	13	NULL	NULL	NULL	statement 5	Process		results from					myofibrils	Cell	addition of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_3_221_s_37	12855672	20 Adrenergic agonists, endothelin-1 (ET-1), and angiotensin II (Ang II) binding to GPCR induce a rather uniform increase in cardiomyocyte size, resulting from the addition of myofibrils in parallel.	bind
22977	8	7275	6	13	NULL	NULL	NULL	statement 6	Process		results from					myofibrils	Cell	addition of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_3_221_s_37	12855672	20 Adrenergic agonists, endothelin-1 (ET-1), and angiotensin II (Ang II) binding to GPCR induce a rather uniform increase in cardiomyocyte size, resulting from the addition of myofibrils in parallel.	bind
46519	9	7275	6	13	NULL	NULL	NULL	ET-1	GP		is a type of					Adrenergic agonist	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_3_221_s_37	12855672	20 Adrenergic agonists, endothelin-1 (ET-1), and angiotensin II (Ang II) binding to GPCR induce a rather uniform increase in cardiomyocyte size, resulting from the addition of myofibrils in parallel.	bind
46520	10	7275	6	13	NULL	NULL	NULL	Ang II	GP		is a type of					Adrenergic agonist	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_3_221_s_37	12855672	20 Adrenergic agonists, endothelin-1 (ET-1), and angiotensin II (Ang II) binding to GPCR induce a rather uniform increase in cardiomyocyte size, resulting from the addition of myofibrils in parallel.	bind
28007	1	7275	7	NULL	NULL	0	NULL	ET-1	NULL		bind	NULL				GPCR	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_93_3_221_s_37	12855672	20 Adrenergic agonists, endothelin-1 (ET-1), and angiotensin II (Ang II) binding to GPCR induce a rather uniform increase in cardiomyocyte size, resulting from the addition of myofibrils in parallel.	bind
28008	2	7275	7	NULL	NULL	0	NULL	Ang II 	NULL		bind	NULL				GPCR	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_93_3_221_s_37	12855672	20 Adrenergic agonists, endothelin-1 (ET-1), and angiotensin II (Ang II) binding to GPCR induce a rather uniform increase in cardiomyocyte size, resulting from the addition of myofibrils in parallel.	bind
28009	3	7275	7	NULL	NULL	0	NULL	statement 1	NULL		induce	NULL				cardiomyocyte size	NULL	increase in			NULL		0	NULL	NULL	NULL	gw60_circulationres_93_3_221_s_37	12855672	20 Adrenergic agonists, endothelin-1 (ET-1), and angiotensin II (Ang II) binding to GPCR induce a rather uniform increase in cardiomyocyte size, resulting from the addition of myofibrils in parallel.	bind
28010	4	7275	7	10	NULL	0	NULL	statement 2			induce					cardiomyocyte size		increase in			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_3_221_s_37	12855672	20 Adrenergic agonists, endothelin-1 (ET-1), and angiotensin II (Ang II) binding to GPCR induce a rather uniform increase in cardiomyocyte size, resulting from the addition of myofibrils in parallel.	bind
28011	5	7275	7	NULL	NULL	0	NULL	ET-1	NULL		is a type of	NULL				Adrenergic agonists	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_93_3_221_s_37	12855672	20 Adrenergic agonists, endothelin-1 (ET-1), and angiotensin II (Ang II) binding to GPCR induce a rather uniform increase in cardiomyocyte size, resulting from the addition of myofibrils in parallel.	bind
28012	6	7275	7	NULL	NULL	0	NULL	Ang II 	NULL		is a type of	NULL				Adrenergic agonists	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_93_3_221_s_37	12855672	20 Adrenergic agonists, endothelin-1 (ET-1), and angiotensin II (Ang II) binding to GPCR induce a rather uniform increase in cardiomyocyte size, resulting from the addition of myofibrils in parallel.	bind
28013	7	7275	7	NULL	NULL	0	NULL	ET-1	NULL		is	NULL				 endothelin-1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_93_3_221_s_37	12855672	20 Adrenergic agonists, endothelin-1 (ET-1), and angiotensin II (Ang II) binding to GPCR induce a rather uniform increase in cardiomyocyte size, resulting from the addition of myofibrils in parallel.	bind
28014	8	7275	7	NULL	NULL	0	NULL	Ang II	NULL		is	NULL				angiotensin II	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_93_3_221_s_37	12855672	20 Adrenergic agonists, endothelin-1 (ET-1), and angiotensin II (Ang II) binding to GPCR induce a rather uniform increase in cardiomyocyte size, resulting from the addition of myofibrils in parallel.	bind
53652	9	7275	7	10	NULL	0	NULL	statement 3			results from					myofibrils		addition of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_3_221_s_37	12855672	20 Adrenergic agonists, endothelin-1 (ET-1), and angiotensin II (Ang II) binding to GPCR induce a rather uniform increase in cardiomyocyte size, resulting from the addition of myofibrils in parallel.	bind
53653	10	7275	7	10	NULL	0	NULL	statement 4			results from					myofibrils 		addition of			NULL		0	NULL	NULL	NULL	gw60_circulationres_93_3_221_s_37	12855672	20 Adrenergic agonists, endothelin-1 (ET-1), and angiotensin II (Ang II) binding to GPCR induce a rather uniform increase in cardiomyocyte size, resulting from the addition of myofibrils in parallel.	bind
23707	1	7276	6	13	NULL	NULL	NULL	fibrils 	CellComponent		is formed by					Abeta	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_128	11549586	20 Although the beta-pleated sheet formation occurring in the fibrils formed by Abeta, hyperphosphorylated tau, as well as alpha-synuclein may be the substrate for BSB and THIOS binding, minor variations in the beta-pleated sheet structures in the lesions described may account for the differences observed in the binding of BSB and THIOS to these lesions.	bind
23708	2	7276	6	13	NULL	NULL	NULL	beta-pleated sheet	GP	formation of	occurs in					statement 1	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_128	11549586	20 Although the beta-pleated sheet formation occurring in the fibrils formed by Abeta, hyperphosphorylated tau, as well as alpha-synuclein may be the substrate for BSB and THIOS binding, minor variations in the beta-pleated sheet structures in the lesions described may account for the differences observed in the binding of BSB and THIOS to these lesions.	bind
23709	3	7276	6	13	NULL	NULL	NULL	tau	GP	hyperphosphorylated	substrate for		may be			BSB	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_128	11549586	20 Although the beta-pleated sheet formation occurring in the fibrils formed by Abeta, hyperphosphorylated tau, as well as alpha-synuclein may be the substrate for BSB and THIOS binding, minor variations in the beta-pleated sheet structures in the lesions described may account for the differences observed in the binding of BSB and THIOS to these lesions.	bind
23710	4	7276	6	13	NULL	NULL	NULL	alpha-synuclein	GP		substrate for		may be			THIOS	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_128	11549586	20 Although the beta-pleated sheet formation occurring in the fibrils formed by Abeta, hyperphosphorylated tau, as well as alpha-synuclein may be the substrate for BSB and THIOS binding, minor variations in the beta-pleated sheet structures in the lesions described may account for the differences observed in the binding of BSB and THIOS to these lesions.	bind
53655	5	7276	6	13	NULL	NULL	NULL	tau	GP	hyperphosphorylated	substrate for		may be			BSB	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_128	11549586	20 Although the beta-pleated sheet formation occurring in the fibrils formed by Abeta, hyperphosphorylated tau, as well as alpha-synuclein may be the substrate for BSB and THIOS binding, minor variations in the beta-pleated sheet structures in the lesions described may account for the differences observed in the binding of BSB and THIOS to these lesions.	bind
53656	6	7276	6	13	NULL	NULL	NULL	alpha-synuclein	GP		substrate for		may be			THIOS	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_128	11549586	20 Although the beta-pleated sheet formation occurring in the fibrils formed by Abeta, hyperphosphorylated tau, as well as alpha-synuclein may be the substrate for BSB and THIOS binding, minor variations in the beta-pleated sheet structures in the lesions described may account for the differences observed in the binding of BSB and THIOS to these lesions.	bind
53657	7	7276	6	13	NULL	NULL	NULL	BSB	Chemical		bind					lesions	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_128	11549586	20 Although the beta-pleated sheet formation occurring in the fibrils formed by Abeta, hyperphosphorylated tau, as well as alpha-synuclein may be the substrate for BSB and THIOS binding, minor variations in the beta-pleated sheet structures in the lesions described may account for the differences observed in the binding of BSB and THIOS to these lesions.	bind
53658	8	7276	6	13	NULL	NULL	NULL	THIOS	Chemical		bind					lesions	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_128	11549586	20 Although the beta-pleated sheet formation occurring in the fibrils formed by Abeta, hyperphosphorylated tau, as well as alpha-synuclein may be the substrate for BSB and THIOS binding, minor variations in the beta-pleated sheet structures in the lesions described may account for the differences observed in the binding of BSB and THIOS to these lesions.	bind
53659	9	7276	6	13	NULL	NULL	NULL	statement 7	Process	differences in	causes					beta-pleated sheet	GP	variations in;;structure of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_128	11549586	20 Although the beta-pleated sheet formation occurring in the fibrils formed by Abeta, hyperphosphorylated tau, as well as alpha-synuclein may be the substrate for BSB and THIOS binding, minor variations in the beta-pleated sheet structures in the lesions described may account for the differences observed in the binding of BSB and THIOS to these lesions.	bind
53660	10	7276	6	13	NULL	NULL	NULL	statement 8	Process	differences in	causes					beta-pleated sheet	GP	variations in;;structure of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_128	11549586	20 Although the beta-pleated sheet formation occurring in the fibrils formed by Abeta, hyperphosphorylated tau, as well as alpha-synuclein may be the substrate for BSB and THIOS binding, minor variations in the beta-pleated sheet structures in the lesions described may account for the differences observed in the binding of BSB and THIOS to these lesions.	bind
28573	1	7276	7	10	NULL	0	NULL	fibrils			is formed by					Abeta					NULL	 	NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_128	11549586	20 Although the beta-pleated sheet formation occurring in the fibrils formed by Abeta, hyperphosphorylated tau, as well as alpha-synuclein may be the substrate for BSB and THIOS binding, minor variations in the beta-pleated sheet structures in the lesions described may account for the differences observed in the binding of BSB and THIOS to these lesions.	bind
28574	2	7276	7	10	NULL	0	NULL	 tau		hyperphosphorylated	 substrate for		may be			BSB		binding of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_128	11549586	20 Although the beta-pleated sheet formation occurring in the fibrils formed by Abeta, hyperphosphorylated tau, as well as alpha-synuclein may be the substrate for BSB and THIOS binding, minor variations in the beta-pleated sheet structures in the lesions described may account for the differences observed in the binding of BSB and THIOS to these lesions.	bind
28575	3	7276	7	10	NULL	0	NULL	alpha-synuclein			substrate for		may be			BSB		binding of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_128	11549586	20 Although the beta-pleated sheet formation occurring in the fibrils formed by Abeta, hyperphosphorylated tau, as well as alpha-synuclein may be the substrate for BSB and THIOS binding, minor variations in the beta-pleated sheet structures in the lesions described may account for the differences observed in the binding of BSB and THIOS to these lesions.	bind
28576	4	7276	7	10	NULL	0	NULL	tau		hyperphosphorylated	substrate for		may be			THIOS		binding of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_128	11549586	20 Although the beta-pleated sheet formation occurring in the fibrils formed by Abeta, hyperphosphorylated tau, as well as alpha-synuclein may be the substrate for BSB and THIOS binding, minor variations in the beta-pleated sheet structures in the lesions described may account for the differences observed in the binding of BSB and THIOS to these lesions.	bind
28577	5	7276	7	10	NULL	0	NULL	alpha-synuclein			substrate for		may be			THIOS		binding of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_128	11549586	20 Although the beta-pleated sheet formation occurring in the fibrils formed by Abeta, hyperphosphorylated tau, as well as alpha-synuclein may be the substrate for BSB and THIOS binding, minor variations in the beta-pleated sheet structures in the lesions described may account for the differences observed in the binding of BSB and THIOS to these lesions.	bind
28578	6	7276	7	NULL	NULL	0	NULL	BSB	NULL		bind	NULL				lesions	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_128	11549586	20 Although the beta-pleated sheet formation occurring in the fibrils formed by Abeta, hyperphosphorylated tau, as well as alpha-synuclein may be the substrate for BSB and THIOS binding, minor variations in the beta-pleated sheet structures in the lesions described may account for the differences observed in the binding of BSB and THIOS to these lesions.	bind
28579	7	7276	7	NULL	NULL	0	NULL	THIOS	NULL		bind	NULL				lesions	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_128	11549586	20 Although the beta-pleated sheet formation occurring in the fibrils formed by Abeta, hyperphosphorylated tau, as well as alpha-synuclein may be the substrate for BSB and THIOS binding, minor variations in the beta-pleated sheet structures in the lesions described may account for the differences observed in the binding of BSB and THIOS to these lesions.	bind
28585	8	7276	7	10	NULL	0	NULL	statement 6		differences in	cause					beta-pleated sheet		variations in;;structure of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_128	11549586	20 Although the beta-pleated sheet formation occurring in the fibrils formed by Abeta, hyperphosphorylated tau, as well as alpha-synuclein may be the substrate for BSB and THIOS binding, minor variations in the beta-pleated sheet structures in the lesions described may account for the differences observed in the binding of BSB and THIOS to these lesions.	bind
28586	9	7276	7	10	NULL	0	NULL	statement 7		differences in	cause					beta-pleated sheet		variations in;;structure of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_128	11549586	20 Although the beta-pleated sheet formation occurring in the fibrils formed by Abeta, hyperphosphorylated tau, as well as alpha-synuclein may be the substrate for BSB and THIOS binding, minor variations in the beta-pleated sheet structures in the lesions described may account for the differences observed in the binding of BSB and THIOS to these lesions.	bind
53654	10	7276	7	10	NULL	0	NULL	beta-pleated sheet		formation of	occurs in					statement 1					NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_128	11549586	20 Although the beta-pleated sheet formation occurring in the fibrils formed by Abeta, hyperphosphorylated tau, as well as alpha-synuclein may be the substrate for BSB and THIOS binding, minor variations in the beta-pleated sheet structures in the lesions described may account for the differences observed in the binding of BSB and THIOS to these lesions.	bind
23134	1	7277	6	13	NULL	NULL	NULL	HSF	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_41_24489_s_79	7592665	20 mM  salicylate  induced HSF DNA binding comparable to a 42  degrees C heat shock,  while lower concentrations produced less HSF DNA binding in a  dose-dependent fashion.	bind
23135	2	7277	6	13	NULL	NULL	NULL	salicylate	Chemical		induces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_41_24489_s_79	7592665	20 mM  salicylate  induced HSF DNA binding comparable to a 42  degrees C heat shock,  while lower concentrations produced less HSF DNA binding in a  dose-dependent fashion.	bind
53661	3	7277	6	13	NULL	NULL	NULL	heat shock			induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_41_24489_s_79	7592665	20 mM  salicylate  induced HSF DNA binding comparable to a 42  degrees C heat shock,  while lower concentrations produced less HSF DNA binding in a  dose-dependent fashion.	bind
53662	4	7277	6	13	NULL	NULL	NULL	statement 2	Process		is comparable to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_41_24489_s_79	7592665	20 mM  salicylate  induced HSF DNA binding comparable to a 42  degrees C heat shock,  while lower concentrations produced less HSF DNA binding in a  dose-dependent fashion.	bind
28587	1	7277	7	NULL	NULL	0	NULL	HSF	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_41_24489_s_79	7592665	20 mM  salicylate  induced HSF DNA binding comparable to a 42  degrees C heat shock,  while lower concentrations produced less HSF DNA binding in a  dose-dependent fashion.	bind
28588	2	7277	7	NULL	NULL	0	NULL	salicylate	NULL		induce	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_41_24489_s_79	7592665	20 mM  salicylate  induced HSF DNA binding comparable to a 42  degrees C heat shock,  while lower concentrations produced less HSF DNA binding in a  dose-dependent fashion.	bind
28589	3	7277	7	NULL	NULL	0	NULL	heat shock	NULL		induce	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_41_24489_s_79	7592665	20 mM  salicylate  induced HSF DNA binding comparable to a 42  degrees C heat shock,  while lower concentrations produced less HSF DNA binding in a  dose-dependent fashion.	bind
28590	4	7277	7	10	NULL	0	NULL	statement 2			is comparable to					statement 3					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_41_24489_s_79	7592665	20 mM  salicylate  induced HSF DNA binding comparable to a 42  degrees C heat shock,  while lower concentrations produced less HSF DNA binding in a  dose-dependent fashion.	bind
23136	1	7280	6	13	NULL	NULL	NULL	p65	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33508_s_181	9837931	20 muM helenalin completely impaired both p65 DNA binding as well as TNF-alpha stimulated NF-kappaB activity.	bind
23137	2	7280	6	13	NULL	NULL	NULL	helenalin	Chemical		impairs		completely			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33508_s_181	9837931	20 muM helenalin completely impaired both p65 DNA binding as well as TNF-alpha stimulated NF-kappaB activity.	bind
23138	3	7280	6	13	NULL	NULL	NULL	TNF-alpha	GP		stimulates					NF-kappaB activity	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33508_s_181	9837931	20 muM helenalin completely impaired both p65 DNA binding as well as TNF-alpha stimulated NF-kappaB activity.	bind
23139	4	7280	6	13	NULL	NULL	NULL	helenalin	Chemical		inhibits		completely			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33508_s_181	9837931	20 muM helenalin completely impaired both p65 DNA binding as well as TNF-alpha stimulated NF-kappaB activity.	bind
28591	1	7280	7	NULL	NULL	0	NULL	 p65	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_50_33508_s_181	9837931	20 muM helenalin completely impaired both p65 DNA binding as well as TNF-alpha stimulated NF-kappaB activity.	bind
28592	2	7280	7	NULL	NULL	0	NULL	helenalin	NULL		impairs	NULL	completely			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33508_s_181	9837931	20 muM helenalin completely impaired both p65 DNA binding as well as TNF-alpha stimulated NF-kappaB activity.	bind
28593	3	7280	7	NULL	NULL	0	NULL	 TNF-alpha	NULL		stimulate	NULL				NF-kappaB	NULL	activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_50_33508_s_181	9837931	20 muM helenalin completely impaired both p65 DNA binding as well as TNF-alpha stimulated NF-kappaB activity.	bind
28594	4	7280	7	NULL	NULL	0	NULL	helenalin	NULL		impairs	NULL	completely			statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_50_33508_s_181	9837931	20 muM helenalin completely impaired both p65 DNA binding as well as TNF-alpha stimulated NF-kappaB activity.	bind
23140	1	7281	6	13	NULL	NULL	NULL	NF-kappaB	GP		activates					transcription	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_10_1585_s_164	11597930	20 Neither has been demonstrated to have a transcription-enhancing property; in fact, activated glucocorticoid responsive element mediates the downregulation of NF-kappaB-activated transcription by interfering with the binding of NF-kappaB p65 to its  cis-element 30 or by directly interfering with transactivation of the NF-kappaB p65 subunit.	bind
23141	2	7281	6	13	NULL	NULL	NULL			activated	mediates				glucocorticoid responsive element	statement 1	Process	downregulation of 			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_10_1585_s_164	11597930	20 Neither has been demonstrated to have a transcription-enhancing property; in fact, activated glucocorticoid responsive element mediates the downregulation of NF-kappaB-activated transcription by interfering with the binding of NF-kappaB p65 to its  cis-element 30 or by directly interfering with transactivation of the NF-kappaB p65 subunit.	bind
23142	3	7281	6	13	NULL	NULL	NULL	NF-kappaB p65	GP		bind									cis-element	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_10_1585_s_164	11597930	20 Neither has been demonstrated to have a transcription-enhancing property; in fact, activated glucocorticoid responsive element mediates the downregulation of NF-kappaB-activated transcription by interfering with the binding of NF-kappaB p65 to its  cis-element 30 or by directly interfering with transactivation of the NF-kappaB p65 subunit.	bind
23143	4	7281	6	13	NULL	NULL	NULL			activated	interfere				glucocorticoid responsive element	statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_10_1585_s_164	11597930	20 Neither has been demonstrated to have a transcription-enhancing property; in fact, activated glucocorticoid responsive element mediates the downregulation of NF-kappaB-activated transcription by interfering with the binding of NF-kappaB p65 to its  cis-element 30 or by directly interfering with transactivation of the NF-kappaB p65 subunit.	bind
23144	5	7281	6	13	NULL	NULL	NULL			activated	interfere		directly		glucocorticoid responsive element	NF-kappaB p65 subunit	GP	transactivation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_10_1585_s_164	11597930	20 Neither has been demonstrated to have a transcription-enhancing property; in fact, activated glucocorticoid responsive element mediates the downregulation of NF-kappaB-activated transcription by interfering with the binding of NF-kappaB p65 to its  cis-element 30 or by directly interfering with transactivation of the NF-kappaB p65 subunit.	bind
23145	6	7281	6	13	NULL	NULL	NULL	statement 2	Process		occurs via					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_10_1585_s_164	11597930	20 Neither has been demonstrated to have a transcription-enhancing property; in fact, activated glucocorticoid responsive element mediates the downregulation of NF-kappaB-activated transcription by interfering with the binding of NF-kappaB p65 to its  cis-element 30 or by directly interfering with transactivation of the NF-kappaB p65 subunit.	bind
53663	7	7281	6	13	NULL	NULL	NULL	statement 2	Process		occur via					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_10_1585_s_164	11597930	20 Neither has been demonstrated to have a transcription-enhancing property; in fact, activated glucocorticoid responsive element mediates the downregulation of NF-kappaB-activated transcription by interfering with the binding of NF-kappaB p65 to its  cis-element 30 or by directly interfering with transactivation of the NF-kappaB p65 subunit.	bind
53664	8	7281	6	13	NULL	NULL	NULL	statement 6	Process		is an alternative to					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_10_1585_s_164	11597930	20 Neither has been demonstrated to have a transcription-enhancing property; in fact, activated glucocorticoid responsive element mediates the downregulation of NF-kappaB-activated transcription by interfering with the binding of NF-kappaB p65 to its  cis-element 30 or by directly interfering with transactivation of the NF-kappaB p65 subunit.	bind
28595	1	7281	7	NULL	NULL	0	NULL	NF-kappaB	NULL		activates	NULL				transcription 	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_10_1585_s_164	11597930	20 Neither has been demonstrated to have a transcription-enhancing property; in fact, activated glucocorticoid responsive element mediates the downregulation of NF-kappaB-activated transcription by interfering with the binding of NF-kappaB p65 to its  cis-element 30 or by directly interfering with transactivation of the NF-kappaB p65 subunit.	bind
28596	2	7281	7	NULL	NULL	0	NULL		NULL	activated	mediates	NULL			glucocorticoid responsive element	statement 1	NULL	downregulation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_10_1585_s_164	11597930	20 Neither has been demonstrated to have a transcription-enhancing property; in fact, activated glucocorticoid responsive element mediates the downregulation of NF-kappaB-activated transcription by interfering with the binding of NF-kappaB p65 to its  cis-element 30 or by directly interfering with transactivation of the NF-kappaB p65 subunit.	bind
28597	3	7281	7	10	NULL	0	NULL	NF-kappaB p65			bind									cis-element	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_10_1585_s_164	11597930	20 Neither has been demonstrated to have a transcription-enhancing property; in fact, activated glucocorticoid responsive element mediates the downregulation of NF-kappaB-activated transcription by interfering with the binding of NF-kappaB p65 to its  cis-element 30 or by directly interfering with transactivation of the NF-kappaB p65 subunit.	bind
28598	4	7281	7	10	NULL	0	NULL			activated	interferes with				glucocorticoid responsive element	statement 3					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_10_1585_s_164	11597930	20 Neither has been demonstrated to have a transcription-enhancing property; in fact, activated glucocorticoid responsive element mediates the downregulation of NF-kappaB-activated transcription by interfering with the binding of NF-kappaB p65 to its  cis-element 30 or by directly interfering with transactivation of the NF-kappaB p65 subunit.	bind
28599	5	7281	7	10	NULL	0	NULL			activated	interferes with				glucocorticoid responsive element	NF-kappaB p65 subunit		transactivation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_10_1585_s_164	11597930	20 Neither has been demonstrated to have a transcription-enhancing property; in fact, activated glucocorticoid responsive element mediates the downregulation of NF-kappaB-activated transcription by interfering with the binding of NF-kappaB p65 to its  cis-element 30 or by directly interfering with transactivation of the NF-kappaB p65 subunit.	bind
28600	6	7281	7	NULL	NULL	0	NULL	statement 2	NULL		occurs by	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_10_1585_s_164	11597930	20 Neither has been demonstrated to have a transcription-enhancing property; in fact, activated glucocorticoid responsive element mediates the downregulation of NF-kappaB-activated transcription by interfering with the binding of NF-kappaB p65 to its  cis-element 30 or by directly interfering with transactivation of the NF-kappaB p65 subunit.	bind
28601	7	7281	7	NULL	NULL	0	NULL	statement 2	NULL		occurs by	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_10_1585_s_164	11597930	20 Neither has been demonstrated to have a transcription-enhancing property; in fact, activated glucocorticoid responsive element mediates the downregulation of NF-kappaB-activated transcription by interfering with the binding of NF-kappaB p65 to its  cis-element 30 or by directly interfering with transactivation of the NF-kappaB p65 subunit.	bind
28602	8	7281	7	NULL	NULL	0	NULL	statement 6	NULL		is an alternative to	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_10_1585_s_164	11597930	20 Neither has been demonstrated to have a transcription-enhancing property; in fact, activated glucocorticoid responsive element mediates the downregulation of NF-kappaB-activated transcription by interfering with the binding of NF-kappaB p65 to its  cis-element 30 or by directly interfering with transactivation of the NF-kappaB p65 subunit.	bind
23146	1	7282	6	13	NULL	NULL	NULL	SCH 23390	Chemical		bind					serotonin 5-HT2 receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_80_4_1187_s_61	9284070	20 nM mianserin was also included to block binding of SCH 23390 to serotonin 5-HT2 receptors for which SCH 23390 has some affinity and which develop early in the rat.	bind
23147	2	7282	6	13	NULL	NULL	NULL	mianserin	Chemical		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_80_4_1187_s_61	9284070	20 nM mianserin was also included to block binding of SCH 23390 to serotonin 5-HT2 receptors for which SCH 23390 has some affinity and which develop early in the rat.	bind
28603	1	7282	7	NULL	NULL	0	NULL	SCH 23390	NULL		bind	NULL				serotonin 5-HT2 receptors	NULL	rat			NULL		0	NULL	NULL	NULL	gw60_neuroscience_80_4_1187_s_61	9284070	20 nM mianserin was also included to block binding of SCH 23390 to serotonin 5-HT2 receptors for which SCH 23390 has some affinity and which develop early in the rat.	bind
28604	2	7282	7	NULL	NULL	0	NULL	mianserin	NULL		blocks	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_neuroscience_80_4_1187_s_61	9284070	20 nM mianserin was also included to block binding of SCH 23390 to serotonin 5-HT2 receptors for which SCH 23390 has some affinity and which develop early in the rat.	bind
23148	1	7283	6	13	NULL	NULL	NULL	eIF2	GP		bind					met-tRNAmet	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_7_926_s_237	15001529	20 One of the critical steps controlling initiation of protein translation is the binding of eukaryotic translation initiation factor 2 (eIF2) to the activated initiator tRNA (met-tRNAmet) and subsequent formation of a ternary complex that binds to the 40S ribosomal subunit.	bind
23149	2	7283	6	13	NULL	NULL	NULL	eIF2	GP		is					eukaryotic translation initiation factor 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_7_926_s_237	15001529	20 One of the critical steps controlling initiation of protein translation is the binding of eukaryotic translation initiation factor 2 (eIF2) to the activated initiator tRNA (met-tRNAmet) and subsequent formation of a ternary complex that binds to the 40S ribosomal subunit.	bind
23150	3	7283	6	13	NULL	NULL	NULL	met-tRNAmet	NucleicAcid		is					activated initiator tRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_7_926_s_237	15001529	20 One of the critical steps controlling initiation of protein translation is the binding of eukaryotic translation initiation factor 2 (eIF2) to the activated initiator tRNA (met-tRNAmet) and subsequent formation of a ternary complex that binds to the 40S ribosomal subunit.	bind
23151	4	7283	6	13	NULL	NULL	NULL	protein translation	Process	initiation of	is controlled by					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_7_926_s_237	15001529	20 One of the critical steps controlling initiation of protein translation is the binding of eukaryotic translation initiation factor 2 (eIF2) to the activated initiator tRNA (met-tRNAmet) and subsequent formation of a ternary complex that binds to the 40S ribosomal subunit.	bind
23152	5	7283	6	13	NULL	NULL	NULL	ternary complex	GP		bind					40S ribosomal subunit	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_7_926_s_237	15001529	20 One of the critical steps controlling initiation of protein translation is the binding of eukaryotic translation initiation factor 2 (eIF2) to the activated initiator tRNA (met-tRNAmet) and subsequent formation of a ternary complex that binds to the 40S ribosomal subunit.	bind
28606	1	7283	7	NULL	NULL	0	NULL	eIF2	NULL		bind	NULL				met-tRNAmet	NULL	activated			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_7_926_s_237	15001529	20 One of the critical steps controlling initiation of protein translation is the binding of eukaryotic translation initiation factor 2 (eIF2) to the activated initiator tRNA (met-tRNAmet) and subsequent formation of a ternary complex that binds to the 40S ribosomal subunit.	bind
28607	2	7283	7	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				ternary complex	NULL	formation of			NULL		0	NULL	NULL	NULL	gw70_circulationres_94_7_926_s_237	15001529	20 One of the critical steps controlling initiation of protein translation is the binding of eukaryotic translation initiation factor 2 (eIF2) to the activated initiator tRNA (met-tRNAmet) and subsequent formation of a ternary complex that binds to the 40S ribosomal subunit.	bind
28608	3	7283	7	NULL	NULL	0	NULL	ternary complex	NULL		binds to	NULL				40S ribosomal subunit	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_7_926_s_237	15001529	20 One of the critical steps controlling initiation of protein translation is the binding of eukaryotic translation initiation factor 2 (eIF2) to the activated initiator tRNA (met-tRNAmet) and subsequent formation of a ternary complex that binds to the 40S ribosomal subunit.	bind
28609	4	7283	7	NULL	NULL	0	NULL	statement 1	NULL		controls	NULL				protein translation	NULL	initiation of			NULL		0	NULL	NULL	NULL	gw70_circulationres_94_7_926_s_237	15001529	20 One of the critical steps controlling initiation of protein translation is the binding of eukaryotic translation initiation factor 2 (eIF2) to the activated initiator tRNA (met-tRNAmet) and subsequent formation of a ternary complex that binds to the 40S ribosomal subunit.	bind
28610	5	7283	7	NULL	NULL	0	NULL	eIF2	NULL		is	NULL				eukaryotic translation initiation factor 2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_7_926_s_237	15001529	20 One of the critical steps controlling initiation of protein translation is the binding of eukaryotic translation initiation factor 2 (eIF2) to the activated initiator tRNA (met-tRNAmet) and subsequent formation of a ternary complex that binds to the 40S ribosomal subunit.	bind
28611	6	7283	7	NULL	NULL	0	NULL	met-tRNAmet	NULL		is	NULL				initiator tRNA	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_7_926_s_237	15001529	20 One of the critical steps controlling initiation of protein translation is the binding of eukaryotic translation initiation factor 2 (eIF2) to the activated initiator tRNA (met-tRNAmet) and subsequent formation of a ternary complex that binds to the 40S ribosomal subunit.	bind
23153	1	7284	6	13	NULL	NULL	NULL	calmodulin	GP		bind					KCNQ1 protein	GP		\tC terminus calmodulin binding motif		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_8_979_s_19	16645144	20 Potential calmodulin binding motifs are found in the KCNQ1 C terminus: accordingly, both the Pongs-Attali group 12 and the Pitt group 13 postulated that calmodulin would bind to the KCNQ1 protein and modulate current amplitude (perhaps even calcium sensitivity).	bind
23154	2	7284	6	13	NULL	NULL	NULL	statement 1	Process		modulate					current amplitude	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_8_979_s_19	16645144	20 Potential calmodulin binding motifs are found in the KCNQ1 C terminus: accordingly, both the Pongs-Attali group 12 and the Pitt group 13 postulated that calmodulin would bind to the KCNQ1 protein and modulate current amplitude (perhaps even calcium sensitivity).	bind
23155	3	7284	6	13	NULL	NULL	NULL	statement 1	Process		modulate		may			calcium sensitivity	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_8_979_s_19	16645144	20 Potential calmodulin binding motifs are found in the KCNQ1 C terminus: accordingly, both the Pongs-Attali group 12 and the Pitt group 13 postulated that calmodulin would bind to the KCNQ1 protein and modulate current amplitude (perhaps even calcium sensitivity).	bind
28612	1	7284	7	NULL	NULL	0	NULL	 calmodulin 	NULL		bind	NULL				KCNQ1 protein	NULL		C terminus calmodulin binding motif		NULL		0	NULL	NULL	NULL	gw70_circulationres_98_8_979_s_19	16645144	20 Potential calmodulin binding motifs are found in the KCNQ1 C terminus: accordingly, both the Pongs-Attali group 12 and the Pitt group 13 postulated that calmodulin would bind to the KCNQ1 protein and modulate current amplitude (perhaps even calcium sensitivity).	bind
28613	2	7284	7	NULL	NULL	0	NULL	statement 1	NULL		modulate	NULL				current amplitude	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_8_979_s_19	16645144	20 Potential calmodulin binding motifs are found in the KCNQ1 C terminus: accordingly, both the Pongs-Attali group 12 and the Pitt group 13 postulated that calmodulin would bind to the KCNQ1 protein and modulate current amplitude (perhaps even calcium sensitivity).	bind
28614	3	7284	7	10	NULL	0	NULL	statement 1			modulate		may			calcium sensitivity					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_8_979_s_19	16645144	20 Potential calmodulin binding motifs are found in the KCNQ1 C terminus: accordingly, both the Pongs-Attali group 12 and the Pitt group 13 postulated that calmodulin would bind to the KCNQ1 protein and modulate current amplitude (perhaps even calcium sensitivity).	bind
23156	1	7285	6	13	NULL	NULL	NULL	caveolin protein	GP		bind					cholesterol	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_9_1528_s_31	12907462	20 The protein caveolin binds cholesterol and stabilizes caveolae.	bind
23157	2	7285	6	13	NULL	NULL	NULL	statement 1	Process		stabilizes					caveolae	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_9_1528_s_31	12907462	20 The protein caveolin binds cholesterol and stabilizes caveolae.	bind
28615	1	7285	7	NULL	NULL	0	NULL	caveolin	NULL		binds	NULL				cholesterol	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_9_1528_s_31	12907462	20 The protein caveolin binds cholesterol and stabilizes caveolae.	bind
28616	2	7285	7	NULL	NULL	0	NULL	statement 1	NULL		stabilize	NULL				caveolae	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_9_1528_s_31	12907462	20 The protein caveolin binds cholesterol and stabilizes caveolae.	bind
23158	1	7286	6	13	NULL	NULL	NULL	Cx43	GP		bind			terminal 5 amino acids (DDLEI)		ZO-1	GP		second PDZ domain		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_3_317_s_39	11861421	20 Together this work has shown that the terminal 5 amino acids (DDLEI) of Cx43 bind the second PDZ domain of ZO-1 and that this interaction may be regulated by src-tyrosine phosphorylation of Cx43.	bind
23159	2	7286	6	13	NULL	NULL	NULL	src	GP		phosphorylates					Cx43	GP		tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_3_317_s_39	11861421	20 Together this work has shown that the terminal 5 amino acids (DDLEI) of Cx43 bind the second PDZ domain of ZO-1 and that this interaction may be regulated by src-tyrosine phosphorylation of Cx43.	bind
23160	3	7286	6	13	NULL	NULL	NULL	statement 2	Process		regulate		may			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_3_317_s_39	11861421	20 Together this work has shown that the terminal 5 amino acids (DDLEI) of Cx43 bind the second PDZ domain of ZO-1 and that this interaction may be regulated by src-tyrosine phosphorylation of Cx43.	bind
28731	1	7286	7	NULL	NULL	0	NULL	Cx43	NULL		bind	NULL		DDLEI		 ZO-1	NULL		PDZ domain		NULL		0	NULL	NULL	NULL	gw60_circulationres_90_3_317_s_39	11861421	20 Together this work has shown that the terminal 5 amino acids (DDLEI) of Cx43 bind the second PDZ domain of ZO-1 and that this interaction may be regulated by src-tyrosine phosphorylation of Cx43.	bind
28732	2	7286	7	NULL	NULL	0	NULL	src	NULL		phosphorylates	NULL				Cx43	NULL		tyrosine		NULL		0	NULL	NULL	NULL	gw60_circulationres_90_3_317_s_39	11861421	20 Together this work has shown that the terminal 5 amino acids (DDLEI) of Cx43 bind the second PDZ domain of ZO-1 and that this interaction may be regulated by src-tyrosine phosphorylation of Cx43.	bind
28733	3	7286	7	NULL	NULL	0	NULL	statement 2	NULL		regulates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_3_317_s_39	11861421	20 Together this work has shown that the terminal 5 amino acids (DDLEI) of Cx43 bind the second PDZ domain of ZO-1 and that this interaction may be regulated by src-tyrosine phosphorylation of Cx43.	bind
23161	1	7287	6	13	NULL	NULL	NULL	RPTPalpha	GP	phosphorylated	bind			tyrosyl		Grb2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_43_41677_s_187	12923167	20% of RPTPalpha is phosphorylated constitutively on Tyr-789 and, like Shp2, tyrosyl-phosphorylated RPTPalpha binds Grb2 ( ,  ).	bind
23162	2	7287	6	13	NULL	NULL	NULL	Shp2	GP	phosphorylated	bind			tyrosyl		Grb2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_43_41677_s_187	12923167	20% of RPTPalpha is phosphorylated constitutively on Tyr-789 and, like Shp2, tyrosyl-phosphorylated RPTPalpha binds Grb2 ( ,  ).	bind
23163	3	7287	6	13	NULL	NULL	NULL	RPTPalpha	GP		is phosphorylated		constitutively						Tyr-789		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_43_41677_s_187	12923167	20% of RPTPalpha is phosphorylated constitutively on Tyr-789 and, like Shp2, tyrosyl-phosphorylated RPTPalpha binds Grb2 ( ,  ).	bind
28734	1	7287	7	NULL	NULL	0	NULL	RPTPalpha	NULL	phosphorylated	binds	NULL		Tyr-789		Grb2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_43_41677_s_187	12923167	20% of RPTPalpha is phosphorylated constitutively on Tyr-789 and, like Shp2, tyrosyl-phosphorylated RPTPalpha binds Grb2 ( ,  ).	bind
28735	2	7287	7	NULL	NULL	0	NULL	RPTPalpha	NULL		phosphorylated 	NULL	constitutively				NULL		Tyr-789		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_43_41677_s_187	12923167	20% of RPTPalpha is phosphorylated constitutively on Tyr-789 and, like Shp2, tyrosyl-phosphorylated RPTPalpha binds Grb2 ( ,  ).	bind
28736	3	7287	7	NULL	NULL	0	NULL	Shp2	NULL	phosphorylated	binds	NULL		tyrosine		Grb2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_43_41677_s_187	12923167	20% of RPTPalpha is phosphorylated constitutively on Tyr-789 and, like Shp2, tyrosyl-phosphorylated RPTPalpha binds Grb2 ( ,  ).	bind
23164	1	7288	6	13	NULL	NULL	NULL	p300	GP		bind					NF-kappaB	GP		RelA (p65) subunit		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_297_s_138	10880399	20, 21  p300 also binds to the RelA (p65) subunit of NF-kappaB and has been shown to be necessary for NF-kappaB-mediated gene transcription.	bind
23165	2	7288	6	13	NULL	NULL	NULL	NF-kappaB	GP		mediates					gene transcription	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_297_s_138	10880399	20, 21  p300 also binds to the RelA (p65) subunit of NF-kappaB and has been shown to be necessary for NF-kappaB-mediated gene transcription.	bind
23166	3	7288	6	13	NULL	NULL	NULL	p300	GP		is necessary for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_297_s_138	10880399	20, 21  p300 also binds to the RelA (p65) subunit of NF-kappaB and has been shown to be necessary for NF-kappaB-mediated gene transcription.	bind
28737	1	7288	7	NULL	NULL	0	NULL	p300	NULL		binds	NULL				NF-kappaB	NULL		RelA (p65) subunit 		NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_1_297_s_138	10880399	20, 21  p300 also binds to the RelA (p65) subunit of NF-kappaB and has been shown to be necessary for NF-kappaB-mediated gene transcription.	bind
28738	2	7288	7	NULL	NULL	0	NULL	NF-kappaB	NULL		mediates	NULL				gene transcription	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_1_297_s_138	10880399	20, 21  p300 also binds to the RelA (p65) subunit of NF-kappaB and has been shown to be necessary for NF-kappaB-mediated gene transcription.	bind
28739	3	7288	7	NULL	NULL	0	NULL	statement 1	NULL		necessary for	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_1_297_s_138	10880399	20, 21  p300 also binds to the RelA (p65) subunit of NF-kappaB and has been shown to be necessary for NF-kappaB-mediated gene transcription.	bind
23167	1	7289	6	13	NULL	NULL	NULL	PDGF-B	GP		bind					HSPG	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_6_512_s_190	16166562	20,107  Binding of PDGF-B to HSPG is most likely needed for localizing secreted PDGF-B in close vicinity to endothelial cells, where it promotes the recognition of PDGFB -  by PDGFR-beta - expressing cells ( Figure 5).	bind
23168	2	7289	6	13	NULL	NULL	NULL	PDGF-B	GP		is localized to					endothelial cells	Cell	close vicinity to			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_6_512_s_190	16166562	20,107  Binding of PDGF-B to HSPG is most likely needed for localizing secreted PDGF-B in close vicinity to endothelial cells, where it promotes the recognition of PDGFB -  by PDGFR-beta - expressing cells ( Figure 5).	bind
23169	3	7289	6	13	NULL	NULL	NULL	statement 1	Process		is needed for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_6_512_s_190	16166562	20,107  Binding of PDGF-B to HSPG is most likely needed for localizing secreted PDGF-B in close vicinity to endothelial cells, where it promotes the recognition of PDGFB -  by PDGFR-beta - expressing cells ( Figure 5).	bind
23170	4	7289	6	13	NULL	NULL	NULL	PDGFR-beta - expressing cells	Cell		recognize					PDGFB	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_6_512_s_190	16166562	20,107  Binding of PDGF-B to HSPG is most likely needed for localizing secreted PDGF-B in close vicinity to endothelial cells, where it promotes the recognition of PDGFB -  by PDGFR-beta - expressing cells ( Figure 5).	bind
23171	5	7289	6	13	NULL	NULL	NULL	PDGF-B	GP		promotes					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_6_512_s_190	16166562	20,107  Binding of PDGF-B to HSPG is most likely needed for localizing secreted PDGF-B in close vicinity to endothelial cells, where it promotes the recognition of PDGFB -  by PDGFR-beta - expressing cells ( Figure 5).	bind
28740	1	7289	7	NULL	NULL	0	NULL	PDGF-B	NULL		bind	NULL				HSPG	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_6_512_s_190	16166562	20,107  Binding of PDGF-B to HSPG is most likely needed for localizing secreted PDGF-B in close vicinity to endothelial cells, where it promotes the recognition of PDGFB -  by PDGFR-beta - expressing cells ( Figure 5).	bind
28741	2	7289	7	NULL	NULL	0	NULL	statement 1	NULL		localize	NULL				PDGF-B	NULL	 secreted 			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_6_512_s_190	16166562	20,107  Binding of PDGF-B to HSPG is most likely needed for localizing secreted PDGF-B in close vicinity to endothelial cells, where it promotes the recognition of PDGFB -  by PDGFR-beta - expressing cells ( Figure 5).	bind
28742	3	7289	7	NULL	NULL	0	NULL	PDGF-B	NULL		is in close vicinity to	NULL				endothelial cells	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_6_512_s_190	16166562	20,107  Binding of PDGF-B to HSPG is most likely needed for localizing secreted PDGF-B in close vicinity to endothelial cells, where it promotes the recognition of PDGFB -  by PDGFR-beta - expressing cells ( Figure 5).	bind
28743	4	7289	7	NULL	NULL	0	NULL	PDGFR-beta - expressing cells	NULL		recognize	NULL				PDGFB	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_6_512_s_190	16166562	20,107  Binding of PDGF-B to HSPG is most likely needed for localizing secreted PDGF-B in close vicinity to endothelial cells, where it promotes the recognition of PDGFB -  by PDGFR-beta - expressing cells ( Figure 5).	bind
28744	5	7289	7	NULL	NULL	0	NULL	statement 3	NULL		promotes	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_6_512_s_190	16166562	20,107  Binding of PDGF-B to HSPG is most likely needed for localizing secreted PDGF-B in close vicinity to endothelial cells, where it promotes the recognition of PDGFB -  by PDGFR-beta - expressing cells ( Figure 5).	bind
23172	1	7290	6	13	NULL	NULL	NULL	glargine	Chemical		has affinity for					IGF-1 receptor	GP				NULL	osteosarcoma cells expressing predominantly IGF-1 receptor	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_325_s_142	14684428	20,21  In osteosarcoma cells expressing predominantly IGF-1 receptors 10 and baby hamster kidney cells overexpressing the human IGF-1 receptor, 10 the affinity of glargine for the IGF-1 receptor is 6- to 8-times higher than that of human insulin, whereas glargine and human insulin bind similarly to cultured human skeletal muscle cells.	bind
23173	2	7290	6	13	NULL	NULL	NULL	glargine	Chemical		has affinity for					IGF-1 receptor	GP				NULL	baby hamster kidney cells overexpressing the human IGF-1 receptor	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_325_s_142	14684428	20,21  In osteosarcoma cells expressing predominantly IGF-1 receptors 10 and baby hamster kidney cells overexpressing the human IGF-1 receptor, 10 the affinity of glargine for the IGF-1 receptor is 6- to 8-times higher than that of human insulin, whereas glargine and human insulin bind similarly to cultured human skeletal muscle cells.	bind
23174	3	7290	6	13	NULL	NULL	NULL	insulin	GP	human	has affinity for					IGF-1 receptor	GP				NULL	osteosarcoma cells expressing predominantly IGF-1 receptor	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_325_s_142	14684428	20,21  In osteosarcoma cells expressing predominantly IGF-1 receptors 10 and baby hamster kidney cells overexpressing the human IGF-1 receptor, 10 the affinity of glargine for the IGF-1 receptor is 6- to 8-times higher than that of human insulin, whereas glargine and human insulin bind similarly to cultured human skeletal muscle cells.	bind
23175	4	7290	6	13	NULL	NULL	NULL	insulin	GP	human	has affinity for					IGF-1 receptor	GP				NULL	baby hamster kidney cells overexpressing the human IGF-1 receptor	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_325_s_142	14684428	20,21  In osteosarcoma cells expressing predominantly IGF-1 receptors 10 and baby hamster kidney cells overexpressing the human IGF-1 receptor, 10 the affinity of glargine for the IGF-1 receptor is 6- to 8-times higher than that of human insulin, whereas glargine and human insulin bind similarly to cultured human skeletal muscle cells.	bind
23176	5	7290	6	13	NULL	NULL	NULL	statement 2	Process	affinity of	is higher than					statement 4	Process	affinity of 			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_325_s_142	14684428	20,21  In osteosarcoma cells expressing predominantly IGF-1 receptors 10 and baby hamster kidney cells overexpressing the human IGF-1 receptor, 10 the affinity of glargine for the IGF-1 receptor is 6- to 8-times higher than that of human insulin, whereas glargine and human insulin bind similarly to cultured human skeletal muscle cells.	bind
23177	6	7290	6	13	NULL	NULL	NULL	glargine	Chemical		bind					IGF-1 receptor	GP				NULL	cultured human skeletal muscle cells	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_325_s_142	14684428	20,21  In osteosarcoma cells expressing predominantly IGF-1 receptors 10 and baby hamster kidney cells overexpressing the human IGF-1 receptor, 10 the affinity of glargine for the IGF-1 receptor is 6- to 8-times higher than that of human insulin, whereas glargine and human insulin bind similarly to cultured human skeletal muscle cells.	bind
46809	7	7290	6	13	NULL	NULL	NULL	statement 1	Process	affinity of	is higher than					statement 3	Process	affinity of 			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_325_s_142	14684428	20,21  In osteosarcoma cells expressing predominantly IGF-1 receptors 10 and baby hamster kidney cells overexpressing the human IGF-1 receptor, 10 the affinity of glargine for the IGF-1 receptor is 6- to 8-times higher than that of human insulin, whereas glargine and human insulin bind similarly to cultured human skeletal muscle cells.	bind
46810	8	7290	6	13	NULL	NULL	NULL	insulin	GP	human	bind					IGF-1 receptor	GP				NULL	cultured human skeletal muscle cells	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_325_s_142	14684428	20,21  In osteosarcoma cells expressing predominantly IGF-1 receptors 10 and baby hamster kidney cells overexpressing the human IGF-1 receptor, 10 the affinity of glargine for the IGF-1 receptor is 6- to 8-times higher than that of human insulin, whereas glargine and human insulin bind similarly to cultured human skeletal muscle cells.	bind
46811	9	7290	6	13	NULL	NULL	NULL	statement 6	Process	affinity of	is similar to					statement 8	Process	affinity of 			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_325_s_142	14684428	20,21  In osteosarcoma cells expressing predominantly IGF-1 receptors 10 and baby hamster kidney cells overexpressing the human IGF-1 receptor, 10 the affinity of glargine for the IGF-1 receptor is 6- to 8-times higher than that of human insulin, whereas glargine and human insulin bind similarly to cultured human skeletal muscle cells.	bind
28745	1	7290	7	NULL	NULL	0	NULL	glargine	NULL		has affinity for	NULL				IGF-1 receptor	NULL				NULL	osteosarcoma cells expressing predominantly IGF-1 receptor	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_325_s_142	14684428	20,21  In osteosarcoma cells expressing predominantly IGF-1 receptors 10 and baby hamster kidney cells overexpressing the human IGF-1 receptor, 10 the affinity of glargine for the IGF-1 receptor is 6- to 8-times higher than that of human insulin, whereas glargine and human insulin bind similarly to cultured human skeletal muscle cells.	bind
28746	2	7290	7	NULL	NULL	0	NULL	glargine	NULL		has affinity for	NULL				IGF-1 receptor	NULL				NULL	baby hamster kidney cells overexpressing the human IGF-1 receptor	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_325_s_142	14684428	20,21  In osteosarcoma cells expressing predominantly IGF-1 receptors 10 and baby hamster kidney cells overexpressing the human IGF-1 receptor, 10 the affinity of glargine for the IGF-1 receptor is 6- to 8-times higher than that of human insulin, whereas glargine and human insulin bind similarly to cultured human skeletal muscle cells.	bind
28747	3	7290	7	NULL	NULL	0	NULL	insulin	NULL	human	has affinity for	NULL				IGF-1 receptor	NULL				NULL	osteosarcoma cells expressing predominantly IGF-1 receptor	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_325_s_142	14684428	20,21  In osteosarcoma cells expressing predominantly IGF-1 receptors 10 and baby hamster kidney cells overexpressing the human IGF-1 receptor, 10 the affinity of glargine for the IGF-1 receptor is 6- to 8-times higher than that of human insulin, whereas glargine and human insulin bind similarly to cultured human skeletal muscle cells.	bind
28748	4	7290	7	NULL	NULL	0	NULL	insulin	NULL	human	has affinity for	NULL				IGF-1 receptor	NULL				NULL	baby hamster kidney cells overexpressing the human IGF-1 receptor	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_325_s_142	14684428	20,21  In osteosarcoma cells expressing predominantly IGF-1 receptors 10 and baby hamster kidney cells overexpressing the human IGF-1 receptor, 10 the affinity of glargine for the IGF-1 receptor is 6- to 8-times higher than that of human insulin, whereas glargine and human insulin bind similarly to cultured human skeletal muscle cells.	bind
28749	5	7290	7	NULL	NULL	0	NULL	statement 1	NULL	affinity of	is higher than	NULL				statement 3	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_325_s_142	14684428	20,21  In osteosarcoma cells expressing predominantly IGF-1 receptors 10 and baby hamster kidney cells overexpressing the human IGF-1 receptor, 10 the affinity of glargine for the IGF-1 receptor is 6- to 8-times higher than that of human insulin, whereas glargine and human insulin bind similarly to cultured human skeletal muscle cells.	bind
28750	6	7290	7	NULL	NULL	0	NULL	statement 2	NULL	affinity of	is higher than	NULL				statement 4	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_325_s_142	14684428	20,21  In osteosarcoma cells expressing predominantly IGF-1 receptors 10 and baby hamster kidney cells overexpressing the human IGF-1 receptor, 10 the affinity of glargine for the IGF-1 receptor is 6- to 8-times higher than that of human insulin, whereas glargine and human insulin bind similarly to cultured human skeletal muscle cells.	bind
28751	7	7290	7	NULL	NULL	0	NULL	glargine	NULL		bind	NULL				IGF-1 receptor	NULL				NULL	cultured human skeletal muscle cells	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_325_s_142	14684428	20,21  In osteosarcoma cells expressing predominantly IGF-1 receptors 10 and baby hamster kidney cells overexpressing the human IGF-1 receptor, 10 the affinity of glargine for the IGF-1 receptor is 6- to 8-times higher than that of human insulin, whereas glargine and human insulin bind similarly to cultured human skeletal muscle cells.	bind
28752	8	7290	7	NULL	NULL	0	NULL	insulin	NULL	human	bind	NULL				IGF-1 receptor	NULL				NULL	cultured human skeletal muscle cells	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_325_s_142	14684428	20,21  In osteosarcoma cells expressing predominantly IGF-1 receptors 10 and baby hamster kidney cells overexpressing the human IGF-1 receptor, 10 the affinity of glargine for the IGF-1 receptor is 6- to 8-times higher than that of human insulin, whereas glargine and human insulin bind similarly to cultured human skeletal muscle cells.	bind
28753	9	7290	7	NULL	NULL	0	NULL	statement 7	NULL		is similar to	NULL				statement 8	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_325_s_142	14684428	20,21  In osteosarcoma cells expressing predominantly IGF-1 receptors 10 and baby hamster kidney cells overexpressing the human IGF-1 receptor, 10 the affinity of glargine for the IGF-1 receptor is 6- to 8-times higher than that of human insulin, whereas glargine and human insulin bind similarly to cultured human skeletal muscle cells.	bind
23178	1	7293	6	13	NULL	NULL	NULL	DRIP Coactivator Complex	GP		bind					vitamin D3 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_2_507_s_672	9430642	20-Epi Analogues of 1,25-Dihydroxyvitamin D3 Are Highly Potent Inducers of DRIP Coactivator Complex Binding to the Vitamin D3 Receptor.	bind
23179	2	7293	6	13	NULL	NULL	NULL	Epi Analogues of 1,25-Dihydroxyvitamin D3	Chemical		induces		highly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_2_507_s_672	9430642	20-Epi Analogues of 1,25-Dihydroxyvitamin D3 Are Highly Potent Inducers of DRIP Coactivator Complex Binding to the Vitamin D3 Receptor.	bind
28754	1	7293	7	NULL	NULL	0	NULL	DRIP Coactivator Complex	NULL		bind	NULL				Vitamin D3 Receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_17_2_507_s_672	9430642	20-Epi Analogues of 1,25-Dihydroxyvitamin D3 Are Highly Potent Inducers of DRIP Coactivator Complex Binding to the Vitamin D3 Receptor.	bind
28755	2	7293	7	10	NULL	0	NULL	Epi Analogues of 1,25-Dihydroxyvitamin D3	NULL		inducers  of	NULL	highly potent			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_2_507_s_672	9430642	20-Epi Analogues of 1,25-Dihydroxyvitamin D3 Are Highly Potent Inducers of DRIP Coactivator Complex Binding to the Vitamin D3 Receptor.	bind
23180	1	7296	6	13	NULL	NULL	NULL	CCh	Chemical		bind					M2 mAChR	GP				NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_312_1_382_s_184	15333678	200-fold reciprocal reduction in ligand affinity when both CCh and gallamine bound to the M2 mAChR at the same time.	bind
23181	2	7296	6	13	NULL	NULL	NULL	gallamine	Chemical		bind					M2 mAChR	GP				NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_312_1_382_s_184	15333678	200-fold reciprocal reduction in ligand affinity when both CCh and gallamine bound to the M2 mAChR at the same time.	bind
23182	3	7296	6	13	NULL	NULL	NULL	statement 1	Process		occurs simultaneously with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_312_1_382_s_184	15333678	200-fold reciprocal reduction in ligand affinity when both CCh and gallamine bound to the M2 mAChR at the same time.	bind
28756	1	7296	7	NULL	NULL	0	NULL	CCh	NULL		bind	NULL				M2 mAChR	NULL				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_312_1_382_s_184	15333678	200-fold reciprocal reduction in ligand affinity when both CCh and gallamine bound to the M2 mAChR at the same time.	bind
28757	2	7296	7	NULL	NULL	0	NULL	gallamine	NULL		bind	NULL				M2 mAChR	NULL				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_312_1_382_s_184	15333678	200-fold reciprocal reduction in ligand affinity when both CCh and gallamine bound to the M2 mAChR at the same time.	bind
28758	3	7296	7	NULL	NULL	0	NULL	statement 1	NULL		occurs simultaneous with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_312_1_382_s_184	15333678	200-fold reciprocal reduction in ligand affinity when both CCh and gallamine bound to the M2 mAChR at the same time.	bind
23183	1	7299	6	13	NULL	NULL	NULL	Mac-2 antigen	Chemical		is					lectin	GP	galactoside specific			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_17_3595_s_319	11522829	21       Cherayil,B.J., Weiner,S.J. and Pillai,S. (1989) The Mac-2 antigen is a galactoside specific lectin that binds IgE.	bind
23184	2	7299	6	13	NULL	NULL	NULL	Mac-2 antigen	Chemical		bind					IgE	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_17_3595_s_319	11522829	21       Cherayil,B.J., Weiner,S.J. and Pillai,S. (1989) The Mac-2 antigen is a galactoside specific lectin that binds IgE.	bind
28759	1	7299	7	NULL	NULL	0	NULL	Mac-2 antigen	NULL		binds	NULL				IgE	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_17_3595_s_319	11522829	21       Cherayil,B.J., Weiner,S.J. and Pillai,S. (1989) The Mac-2 antigen is a galactoside specific lectin that binds IgE.	bind
28760	2	7299	7	NULL	NULL	0	NULL	Mac-2 antigen	NULL		is a type of	NULL				galactoside specific lectin	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_17_3595_s_319	11522829	21       Cherayil,B.J., Weiner,S.J. and Pillai,S. (1989) The Mac-2 antigen is a galactoside specific lectin that binds IgE.	bind
23185	1	7300	6	13	NULL	NULL	NULL	tRNALys molecule	NucleicAcid		plays a role in					reverse transcription	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2757_s_315	11433020	21       Das,A.T., Klaver,B. and Berkhout,B. (1997) Sequence variation of the HIV primer binding site suggests the use of an alternative tRNALys molecule in reverse transcription.	bind
23186	2	7300	6	13	NULL	NULL	NULL	HIV 	NucleicAcid	sequence variation of 	suggests				primer binding site	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2757_s_315	11433020	21       Das,A.T., Klaver,B. and Berkhout,B. (1997) Sequence variation of the HIV primer binding site suggests the use of an alternative tRNALys molecule in reverse transcription.	bind
28761	1	7300	7	NULL	NULL	0	NULL	tRNALys molecule	NULL		is involved in	NULL				reverse transcription	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2757_s_315	11433020	21       Das,A.T., Klaver,B. and Berkhout,B. (1997) Sequence variation of the HIV primer binding site suggests the use of an alternative tRNALys molecule in reverse transcription.	bind
54469	2	7300	7	10	NULL	0	NULL	HIV		sequence variation of 	suggest				primer binding site	statement 1					NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2757_s_315	11433020	21       Das,A.T., Klaver,B. and Berkhout,B. (1997) Sequence variation of the HIV primer binding site suggests the use of an alternative tRNALys molecule in reverse transcription.	bind
26420	1	7302	5	13	NULL	NULL	NULL	spermine	Chemical		bind					B-DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_5121_s_285	11812845	21       Tari,L.W. and Secco,A.S. (1995) Base-pair opening and spermine binding B-DNA features displayed in the crystal structure of a gal operon fragment: implications for protein-DNA recognition.	bind
28762	1	7302	7	NULL	NULL	0	NULL	spermine	NULL		bind	NULL				B-DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_5121_s_285	11812845	21       Tari,L.W. and Secco,A.S. (1995) Base-pair opening and spermine binding B-DNA features displayed in the crystal structure of a gal operon fragment: implications for protein-DNA recognition.	bind
26421	1	7303	5	13	NULL	NULL	NULL	GP Ib/VIX	GP		bind					vWF	GP		A1 domain		NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_4_437_s_50	10421606	21  GP Ib/VIX binding to the A1 domain is facilitated when vWF becomes activated either by its binding to collagen on vessel walls or by conditions of high shear.	bind
26422	2	7303	5	13	NULL	NULL	NULL	vWF	GP		bind					collagen	GP				NULL	on vessel walls	NULL	NULL	NULL	NULL	gw60_circulation_100_4_437_s_50	10421606	21  GP Ib/VIX binding to the A1 domain is facilitated when vWF becomes activated either by its binding to collagen on vessel walls or by conditions of high shear.	bind
26423	3	7303	5	13	NULL	NULL	NULL	statement 2	Process		activates					vWF	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_4_437_s_50	10421606	21  GP Ib/VIX binding to the A1 domain is facilitated when vWF becomes activated either by its binding to collagen on vessel walls or by conditions of high shear.	bind
26424	4	7303	5	13	NULL	NULL	NULL	shear		high	activates					vWF	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_4_437_s_50	10421606	21  GP Ib/VIX binding to the A1 domain is facilitated when vWF becomes activated either by its binding to collagen on vessel walls or by conditions of high shear.	bind
26425	5	7303	5	13	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_4_437_s_50	10421606	21  GP Ib/VIX binding to the A1 domain is facilitated when vWF becomes activated either by its binding to collagen on vessel walls or by conditions of high shear.	bind
26426	6	7303	5	13	NULL	NULL	NULL	statement 3	Process		facilitates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_4_437_s_50	10421606	21  GP Ib/VIX binding to the A1 domain is facilitated when vWF becomes activated either by its binding to collagen on vessel walls or by conditions of high shear.	bind
26427	7	7303	5	13	NULL	NULL	NULL	statement 4	Process		facilitates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_4_437_s_50	10421606	21  GP Ib/VIX binding to the A1 domain is facilitated when vWF becomes activated either by its binding to collagen on vessel walls or by conditions of high shear.	bind
28763	1	7303	7	10	NULL	0	NULL	GP Ib/VIX			binds to					vWF			A1 domain		NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_4_437_s_50	10421606	21  GP Ib/VIX binding to the A1 domain is facilitated when vWF becomes activated either by its binding to collagen on vessel walls or by conditions of high shear.	bind
28764	2	7303	7	NULL	NULL	0	NULL	vWF	NULL		bind	NULL				collagen	NULL				NULL	vessel walls	0	NULL	NULL	NULL	gw60_circulation_100_4_437_s_50	10421606	21  GP Ib/VIX binding to the A1 domain is facilitated when vWF becomes activated either by its binding to collagen on vessel walls or by conditions of high shear.	bind
28765	3	7303	7	NULL	NULL	0	NULL	statement 2	NULL		activates	NULL				vWF	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_100_4_437_s_50	10421606	21  GP Ib/VIX binding to the A1 domain is facilitated when vWF becomes activated either by its binding to collagen on vessel walls or by conditions of high shear.	bind
28766	4	7303	7	10	NULL	0	NULL	shear		high	activates					vWF					NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_4_437_s_50	10421606	21  GP Ib/VIX binding to the A1 domain is facilitated when vWF becomes activated either by its binding to collagen on vessel walls or by conditions of high shear.	bind
28767	5	7303	7	NULL	NULL	0	NULL	statement 3	NULL		facilitates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_100_4_437_s_50	10421606	21  GP Ib/VIX binding to the A1 domain is facilitated when vWF becomes activated either by its binding to collagen on vessel walls or by conditions of high shear.	bind
28768	6	7303	7	NULL	NULL	0	NULL	statement 4	NULL		facilitates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_100_4_437_s_50	10421606	21  GP Ib/VIX binding to the A1 domain is facilitated when vWF becomes activated either by its binding to collagen on vessel walls or by conditions of high shear.	bind
54470	7	7303	7	10	NULL	0	NULL	statement 3			is an alternative to					statement 4					NULL		0	NULL	NULL	NULL	gw60_circulation_100_4_437_s_50	10421606	21  GP Ib/VIX binding to the A1 domain is facilitated when vWF becomes activated either by its binding to collagen on vessel walls or by conditions of high shear.	bind
26428	1	7305	5	13	NULL	NULL	NULL	WGA	GP		bind					endothelial cells	Cell	luminal surface of			NULL	in arterioles	NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1099_s_215	9777941	21  In tracheal vessels of pathogen-free C3H and C57BL/6 mice, WGA bound to the luminal surface of endothelial cells in arterioles and capillaries but bound weakly or not at all in venules (Figure 8A)   .	bind
26429	2	7305	5	13	NULL	NULL	NULL	WGA	GP		bind					endothelial cells	Cell	luminal surface of			NULL	in capillaries	NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1099_s_215	9777941	21  In tracheal vessels of pathogen-free C3H and C57BL/6 mice, WGA bound to the luminal surface of endothelial cells in arterioles and capillaries but bound weakly or not at all in venules (Figure 8A)   .	bind
26430	3	7305	5	13	NULL	NULL	NULL	statement 1	Process		occurs in					tracheal vessels	OrganismPart				NULL	in pathogen-free C3H mice	NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1099_s_215	9777941	21  In tracheal vessels of pathogen-free C3H and C57BL/6 mice, WGA bound to the luminal surface of endothelial cells in arterioles and capillaries but bound weakly or not at all in venules (Figure 8A)   .	bind
26431	4	7305	5	13	NULL	NULL	NULL	statement 1	Process		occurs in					tracheal vessels	OrganismPart				NULL	in pathogen-free C57BL/6 mice	NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1099_s_215	9777941	21  In tracheal vessels of pathogen-free C3H and C57BL/6 mice, WGA bound to the luminal surface of endothelial cells in arterioles and capillaries but bound weakly or not at all in venules (Figure 8A)   .	bind
26432	5	7305	5	13	NULL	NULL	NULL	statement 2	Process		occurs in					tracheal vessels	OrganismPart				NULL	in pathogen-free C3H mice	NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1099_s_215	9777941	21  In tracheal vessels of pathogen-free C3H and C57BL/6 mice, WGA bound to the luminal surface of endothelial cells in arterioles and capillaries but bound weakly or not at all in venules (Figure 8A)   .	bind
26433	6	7305	5	13	NULL	NULL	NULL	statement 2	Process		occurs in					tracheal vessels	OrganismPart				NULL	in pathogen-free C57BL/6 mice	NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1099_s_215	9777941	21  In tracheal vessels of pathogen-free C3H and C57BL/6 mice, WGA bound to the luminal surface of endothelial cells in arterioles and capillaries but bound weakly or not at all in venules (Figure 8A)   .	bind
26434	7	7305	5	13	NULL	NULL	NULL	WGA	GP		bind		weakly			endothelial cells	Cell	luminal surface of			NULL	in venules	NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1099_s_215	9777941	21  In tracheal vessels of pathogen-free C3H and C57BL/6 mice, WGA bound to the luminal surface of endothelial cells in arterioles and capillaries but bound weakly or not at all in venules (Figure 8A)   .	bind
26435	8	7305	5	13	NULL	NULL	NULL	statement 7	Process		occurs in					tracheal vessels	OrganismPart				NULL	in pathogen-free C3H mice	NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1099_s_215	9777941	21  In tracheal vessels of pathogen-free C3H and C57BL/6 mice, WGA bound to the luminal surface of endothelial cells in arterioles and capillaries but bound weakly or not at all in venules (Figure 8A)   .	bind
26436	9	7305	5	13	NULL	NULL	NULL	statement 7	Process		occurs in					tracheal vessels	OrganismPart				NULL	in pathogen-free C57BL/6 mice	NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1099_s_215	9777941	21  In tracheal vessels of pathogen-free C3H and C57BL/6 mice, WGA bound to the luminal surface of endothelial cells in arterioles and capillaries but bound weakly or not at all in venules (Figure 8A)   .	bind
28769	1	7305	7	NULL	NULL	0	NULL	WGA			bind					endothelial cells 		luminal surface of 			NULL	arterioles	NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1099_s_215	9777941	21  In tracheal vessels of pathogen-free C3H and C57BL/6 mice, WGA bound to the luminal surface of endothelial cells in arterioles and capillaries but bound weakly or not at all in venules (Figure 8A)   .	bind
28770	2	7305	7	NULL	NULL	0	NULL	WGA			bind					endothelial cells 		luminal surface of 			NULL	capillaries	NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1099_s_215	9777941	21  In tracheal vessels of pathogen-free C3H and C57BL/6 mice, WGA bound to the luminal surface of endothelial cells in arterioles and capillaries but bound weakly or not at all in venules (Figure 8A)   .	bind
28771	3	7305	7	NULL	NULL	0	NULL	WGA			bind		weakly			endothelial cells		luminal surface of 			NULL	venules	NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1099_s_215	9777941	21  In tracheal vessels of pathogen-free C3H and C57BL/6 mice, WGA bound to the luminal surface of endothelial cells in arterioles and capillaries but bound weakly or not at all in venules (Figure 8A)   .	bind
28772	4	7305	7	NULL	NULL	0	NULL	WGA			does not bind					endothelial cells		luminal surface of			NULL	venules	NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1099_s_215	9777941	21  In tracheal vessels of pathogen-free C3H and C57BL/6 mice, WGA bound to the luminal surface of endothelial cells in arterioles and capillaries but bound weakly or not at all in venules (Figure 8A)   .	bind
28773	5	7305	7	NULL	NULL	0	NULL	statement 1			occur in					 pathogen-free C3H mice		tracheal vessels of 			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1099_s_215	9777941	21  In tracheal vessels of pathogen-free C3H and C57BL/6 mice, WGA bound to the luminal surface of endothelial cells in arterioles and capillaries but bound weakly or not at all in venules (Figure 8A)   .	bind
28774	6	7305	7	NULL	NULL	0	NULL	statement 1			occur in					  C57BL/6 mice		tracheal vessels of 			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1099_s_215	9777941	21  In tracheal vessels of pathogen-free C3H and C57BL/6 mice, WGA bound to the luminal surface of endothelial cells in arterioles and capillaries but bound weakly or not at all in venules (Figure 8A)   .	bind
28775	7	7305	7	NULL	NULL	0	NULL	statement 2			occur in					pathogen-free C3H mice		tracheal vessels of 			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1099_s_215	9777941	21  In tracheal vessels of pathogen-free C3H and C57BL/6 mice, WGA bound to the luminal surface of endothelial cells in arterioles and capillaries but bound weakly or not at all in venules (Figure 8A)   .	bind
28776	8	7305	7	NULL	NULL	0	NULL	statement 2			occur in					C57BL/6 mice		tracheal vessels of 			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1099_s_215	9777941	21  In tracheal vessels of pathogen-free C3H and C57BL/6 mice, WGA bound to the luminal surface of endothelial cells in arterioles and capillaries but bound weakly or not at all in venules (Figure 8A)   .	bind
54671	9	7305	7	NULL	NULL	0	NULL	statement 3			occur in					pathogen-free C3H mice		tracheal vessels of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_4_1099_s_215	9777941	21  In tracheal vessels of pathogen-free C3H and C57BL/6 mice, WGA bound to the luminal surface of endothelial cells in arterioles and capillaries but bound weakly or not at all in venules (Figure 8A)   .	bind
54672	10	7305	7	NULL	NULL	0	NULL	statement 3			occur in					C57BL/6 mice		tracheal vessels of 			NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_4_1099_s_215	9777941	21  In tracheal vessels of pathogen-free C3H and C57BL/6 mice, WGA bound to the luminal surface of endothelial cells in arterioles and capillaries but bound weakly or not at all in venules (Figure 8A)   .	bind
54673	11	7305	7	NULL	NULL	0	NULL	statement 4			occur in					pathogen-free C3H mice		tracheal vessels of 			NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_4_1099_s_215	9777941	21  In tracheal vessels of pathogen-free C3H and C57BL/6 mice, WGA bound to the luminal surface of endothelial cells in arterioles and capillaries but bound weakly or not at all in venules (Figure 8A)   .	bind
54674	12	7305	7	NULL	NULL	0	NULL	statement 4			occur in					C57BL/6 mice		tracheal vessels of 			NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_4_1099_s_215	9777941	21  In tracheal vessels of pathogen-free C3H and C57BL/6 mice, WGA bound to the luminal surface of endothelial cells in arterioles and capillaries but bound weakly or not at all in venules (Figure 8A)   .	bind
54675	13	7305	7	NULL	NULL	0	NULL	statement 3			is an alternative to					statement 4					NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_4_1099_s_215	9777941	21  In tracheal vessels of pathogen-free C3H and C57BL/6 mice, WGA bound to the luminal surface of endothelial cells in arterioles and capillaries but bound weakly or not at all in venules (Figure 8A)   .	bind
26437	1	7306	5	13	NULL	NULL	NULL	VCAM-1 immunoglobulin	GP		bind					peripheral T cells	Cell	resting 			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_723_s_237	9598830	21  Jakubowski et al 39  reported that there was little binding of VCAM-1 immunoglobulin to resting peripheral T cells even at a concentration of 100 mug/mL, whereas VCAM-1 immunoglobulin at a concentration as low as 0.03 mug/mL bound to T cells stimulated with MnCl2.	bind
26438	2	7306	5	13	NULL	NULL	NULL	T cells	Cell		is stimulated with					MnCl2	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_723_s_237	9598830	21  Jakubowski et al 39  reported that there was little binding of VCAM-1 immunoglobulin to resting peripheral T cells even at a concentration of 100 mug/mL, whereas VCAM-1 immunoglobulin at a concentration as low as 0.03 mug/mL bound to T cells stimulated with MnCl2.	bind
26439	3	7306	5	13	NULL	NULL	NULL	VCAM-1 immunoglobulin	GP		bind					statement 2	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_723_s_237	9598830	21  Jakubowski et al 39  reported that there was little binding of VCAM-1 immunoglobulin to resting peripheral T cells even at a concentration of 100 mug/mL, whereas VCAM-1 immunoglobulin at a concentration as low as 0.03 mug/mL bound to T cells stimulated with MnCl2.	bind
28777	1	7306	7	NULL	NULL	0	NULL	VCAM-1 immunoglobulin	NULL		bind	NULL	less			peripheral T cells	NULL	resting			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_723_s_237	9598830	21  Jakubowski et al 39  reported that there was little binding of VCAM-1 immunoglobulin to resting peripheral T cells even at a concentration of 100 mug/mL, whereas VCAM-1 immunoglobulin at a concentration as low as 0.03 mug/mL bound to T cells stimulated with MnCl2.	bind
28778	2	7306	7	NULL	NULL	0	NULL	Mncl2	NULL		stimulates	NULL				T cells	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_723_s_237	9598830	21  Jakubowski et al 39  reported that there was little binding of VCAM-1 immunoglobulin to resting peripheral T cells even at a concentration of 100 mug/mL, whereas VCAM-1 immunoglobulin at a concentration as low as 0.03 mug/mL bound to T cells stimulated with MnCl2.	bind
28779	3	7306	7	NULL	NULL	0	NULL	VCAM-1 immunoglobulin	NULL		bind	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_723_s_237	9598830	21  Jakubowski et al 39  reported that there was little binding of VCAM-1 immunoglobulin to resting peripheral T cells even at a concentration of 100 mug/mL, whereas VCAM-1 immunoglobulin at a concentration as low as 0.03 mug/mL bound to T cells stimulated with MnCl2.	bind
28993	1	7307	5	13	NULL	NULL	NULL	ASA	Chemical		blocks					cyclooxygenase	GP	platelet			NULL		NULL	NULL	NULL	NULL	gw60_circulation_93_6_1201_s_129	8653842	21  The aggregation response to shear forces generated in a cone and plate viscometer showed that neither the mobilization of cytosolic Ca2+ nor the aggregation response to shear stress was inhibited by blocking the platelet cyclooxygenase and thromboxane A2 production with ASA. 22  These results suggest that the high levels of shear stress (>30 dyne/cm2) may have induced plasma vWF to bind to platelet GPIb and caused an increase in platelet cytosolic Ca2+ and platelet aggregation, both of which are potentiated by the vWF binding to the platelet GPIIb-IIIa complex.	bind
28994	2	7307	5	13	NULL	NULL	NULL	ASA	Chemical		blocks					thromboxane A2	Chemical	production of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_93_6_1201_s_129	8653842	21  The aggregation response to shear forces generated in a cone and plate viscometer showed that neither the mobilization of cytosolic Ca2+ nor the aggregation response to shear stress was inhibited by blocking the platelet cyclooxygenase and thromboxane A2 production with ASA. 22  These results suggest that the high levels of shear stress (>30 dyne/cm2) may have induced plasma vWF to bind to platelet GPIb and caused an increase in platelet cytosolic Ca2+ and platelet aggregation, both of which are potentiated by the vWF binding to the platelet GPIIb-IIIa complex.	bind
28995	3	7307	5	13	NULL	NULL	NULL	statement 1	Process		does not inhibit					cytosolic Ca2+	Chemical	mobilization of 			NULL		NULL	NULL	NULL	NULL	gw60_circulation_93_6_1201_s_129	8653842	21  The aggregation response to shear forces generated in a cone and plate viscometer showed that neither the mobilization of cytosolic Ca2+ nor the aggregation response to shear stress was inhibited by blocking the platelet cyclooxygenase and thromboxane A2 production with ASA. 22  These results suggest that the high levels of shear stress (>30 dyne/cm2) may have induced plasma vWF to bind to platelet GPIb and caused an increase in platelet cytosolic Ca2+ and platelet aggregation, both of which are potentiated by the vWF binding to the platelet GPIIb-IIIa complex.	bind
28996	4	7307	5	13	NULL	NULL	NULL	statement 2	Process		does not inhibit					cytosolic Ca2+	Chemical	mobilization of 			NULL		NULL	NULL	NULL	NULL	gw60_circulation_93_6_1201_s_129	8653842	21  The aggregation response to shear forces generated in a cone and plate viscometer showed that neither the mobilization of cytosolic Ca2+ nor the aggregation response to shear stress was inhibited by blocking the platelet cyclooxygenase and thromboxane A2 production with ASA. 22  These results suggest that the high levels of shear stress (>30 dyne/cm2) may have induced plasma vWF to bind to platelet GPIb and caused an increase in platelet cytosolic Ca2+ and platelet aggregation, both of which are potentiated by the vWF binding to the platelet GPIIb-IIIa complex.	bind
28997	5	7307	5	13	NULL	NULL	NULL	shear stress			induce					aggregation	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_93_6_1201_s_129	8653842	21  The aggregation response to shear forces generated in a cone and plate viscometer showed that neither the mobilization of cytosolic Ca2+ nor the aggregation response to shear stress was inhibited by blocking the platelet cyclooxygenase and thromboxane A2 production with ASA. 22  These results suggest that the high levels of shear stress (>30 dyne/cm2) may have induced plasma vWF to bind to platelet GPIb and caused an increase in platelet cytosolic Ca2+ and platelet aggregation, both of which are potentiated by the vWF binding to the platelet GPIIb-IIIa complex.	bind
28998	6	7307	5	13	NULL	NULL	NULL	statement 1	Process		does not inhibit					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_93_6_1201_s_129	8653842	21  The aggregation response to shear forces generated in a cone and plate viscometer showed that neither the mobilization of cytosolic Ca2+ nor the aggregation response to shear stress was inhibited by blocking the platelet cyclooxygenase and thromboxane A2 production with ASA. 22  These results suggest that the high levels of shear stress (>30 dyne/cm2) may have induced plasma vWF to bind to platelet GPIb and caused an increase in platelet cytosolic Ca2+ and platelet aggregation, both of which are potentiated by the vWF binding to the platelet GPIIb-IIIa complex.	bind
28999	7	7307	5	13	NULL	NULL	NULL	statement 2	Process		does not inhibit					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_93_6_1201_s_129	8653842	21  The aggregation response to shear forces generated in a cone and plate viscometer showed that neither the mobilization of cytosolic Ca2+ nor the aggregation response to shear stress was inhibited by blocking the platelet cyclooxygenase and thromboxane A2 production with ASA. 22  These results suggest that the high levels of shear stress (>30 dyne/cm2) may have induced plasma vWF to bind to platelet GPIb and caused an increase in platelet cytosolic Ca2+ and platelet aggregation, both of which are potentiated by the vWF binding to the platelet GPIIb-IIIa complex.	bind
29000	8	7307	5	13	NULL	NULL	NULL	vWF	GP	plasma	bind					GPIb	GP	platelet			NULL		NULL	NULL	NULL	NULL	gw60_circulation_93_6_1201_s_129	8653842	21  The aggregation response to shear forces generated in a cone and plate viscometer showed that neither the mobilization of cytosolic Ca2+ nor the aggregation response to shear stress was inhibited by blocking the platelet cyclooxygenase and thromboxane A2 production with ASA. 22  These results suggest that the high levels of shear stress (>30 dyne/cm2) may have induced plasma vWF to bind to platelet GPIb and caused an increase in platelet cytosolic Ca2+ and platelet aggregation, both of which are potentiated by the vWF binding to the platelet GPIIb-IIIa complex.	bind
29001	9	7307	5	13	NULL	NULL	NULL	shear stress		high levels of	induces		may			statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_93_6_1201_s_129	8653842	21  The aggregation response to shear forces generated in a cone and plate viscometer showed that neither the mobilization of cytosolic Ca2+ nor the aggregation response to shear stress was inhibited by blocking the platelet cyclooxygenase and thromboxane A2 production with ASA. 22  These results suggest that the high levels of shear stress (>30 dyne/cm2) may have induced plasma vWF to bind to platelet GPIb and caused an increase in platelet cytosolic Ca2+ and platelet aggregation, both of which are potentiated by the vWF binding to the platelet GPIIb-IIIa complex.	bind
29002	10	7307	5	13	NULL	NULL	NULL	shear stress		high levels of	increases					cytosolic Ca2+	Chemical	platelet			NULL		NULL	NULL	NULL	NULL	gw60_circulation_93_6_1201_s_129	8653842	21  The aggregation response to shear forces generated in a cone and plate viscometer showed that neither the mobilization of cytosolic Ca2+ nor the aggregation response to shear stress was inhibited by blocking the platelet cyclooxygenase and thromboxane A2 production with ASA. 22  These results suggest that the high levels of shear stress (>30 dyne/cm2) may have induced plasma vWF to bind to platelet GPIb and caused an increase in platelet cytosolic Ca2+ and platelet aggregation, both of which are potentiated by the vWF binding to the platelet GPIIb-IIIa complex.	bind
29003	11	7307	5	13	NULL	NULL	NULL	shear stress		high levels of	increases					platelets	Cell	aggregation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_93_6_1201_s_129	8653842	21  The aggregation response to shear forces generated in a cone and plate viscometer showed that neither the mobilization of cytosolic Ca2+ nor the aggregation response to shear stress was inhibited by blocking the platelet cyclooxygenase and thromboxane A2 production with ASA. 22  These results suggest that the high levels of shear stress (>30 dyne/cm2) may have induced plasma vWF to bind to platelet GPIb and caused an increase in platelet cytosolic Ca2+ and platelet aggregation, both of which are potentiated by the vWF binding to the platelet GPIIb-IIIa complex.	bind
29004	12	7307	5	13	NULL	NULL	NULL	vWF	GP		bind					GPIIb-IIIa complex	GP	platelet			NULL		NULL	NULL	NULL	NULL	gw60_circulation_93_6_1201_s_129	8653842	21  The aggregation response to shear forces generated in a cone and plate viscometer showed that neither the mobilization of cytosolic Ca2+ nor the aggregation response to shear stress was inhibited by blocking the platelet cyclooxygenase and thromboxane A2 production with ASA. 22  These results suggest that the high levels of shear stress (>30 dyne/cm2) may have induced plasma vWF to bind to platelet GPIb and caused an increase in platelet cytosolic Ca2+ and platelet aggregation, both of which are potentiated by the vWF binding to the platelet GPIIb-IIIa complex.	bind
29005	13	7307	5	13	NULL	NULL	NULL	statement 12	Process		potentiate					statement 10	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_93_6_1201_s_129	8653842	21  The aggregation response to shear forces generated in a cone and plate viscometer showed that neither the mobilization of cytosolic Ca2+ nor the aggregation response to shear stress was inhibited by blocking the platelet cyclooxygenase and thromboxane A2 production with ASA. 22  These results suggest that the high levels of shear stress (>30 dyne/cm2) may have induced plasma vWF to bind to platelet GPIb and caused an increase in platelet cytosolic Ca2+ and platelet aggregation, both of which are potentiated by the vWF binding to the platelet GPIIb-IIIa complex.	bind
29006	14	7307	5	13	NULL	NULL	NULL	statement 12	Process		potentiate					statement 11	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_93_6_1201_s_129	8653842	21  The aggregation response to shear forces generated in a cone and plate viscometer showed that neither the mobilization of cytosolic Ca2+ nor the aggregation response to shear stress was inhibited by blocking the platelet cyclooxygenase and thromboxane A2 production with ASA. 22  These results suggest that the high levels of shear stress (>30 dyne/cm2) may have induced plasma vWF to bind to platelet GPIb and caused an increase in platelet cytosolic Ca2+ and platelet aggregation, both of which are potentiated by the vWF binding to the platelet GPIIb-IIIa complex.	bind
28780	1	7307	7	10	NULL	0	NULL	ASA			blocks					cyclooxygenase		production of;;platelet			NULL		NULL	NULL	NULL	NULL	gw60_circulation_93_6_1201_s_129	8653842	21  The aggregation response to shear forces generated in a cone and plate viscometer showed that neither the mobilization of cytosolic Ca2+ nor the aggregation response to shear stress was inhibited by blocking the platelet cyclooxygenase and thromboxane A2 production with ASA. 22  These results suggest that the high levels of shear stress (>30 dyne/cm2) may have induced plasma vWF to bind to platelet GPIb and caused an increase in platelet cytosolic Ca2+ and platelet aggregation, both of which are potentiated by the vWF binding to the platelet GPIIb-IIIa complex.	bind
28781	2	7307	7	NULL	NULL	0	NULL	ASA	NULL		blocks	NULL				thromboxane A2	NULL	production of			NULL		0	NULL	NULL	NULL	gw60_circulation_93_6_1201_s_129	8653842	21  The aggregation response to shear forces generated in a cone and plate viscometer showed that neither the mobilization of cytosolic Ca2+ nor the aggregation response to shear stress was inhibited by blocking the platelet cyclooxygenase and thromboxane A2 production with ASA. 22  These results suggest that the high levels of shear stress (>30 dyne/cm2) may have induced plasma vWF to bind to platelet GPIb and caused an increase in platelet cytosolic Ca2+ and platelet aggregation, both of which are potentiated by the vWF binding to the platelet GPIIb-IIIa complex.	bind
28782	3	7307	7	10	NULL	0	NULL	statement 1	NULL		does not inhibit	NULL				cytosolic Ca2+	NULL	mobilization of 			NULL		NULL	NULL	NULL	NULL	gw60_circulation_93_6_1201_s_129	8653842	21  The aggregation response to shear forces generated in a cone and plate viscometer showed that neither the mobilization of cytosolic Ca2+ nor the aggregation response to shear stress was inhibited by blocking the platelet cyclooxygenase and thromboxane A2 production with ASA. 22  These results suggest that the high levels of shear stress (>30 dyne/cm2) may have induced plasma vWF to bind to platelet GPIb and caused an increase in platelet cytosolic Ca2+ and platelet aggregation, both of which are potentiated by the vWF binding to the platelet GPIIb-IIIa complex.	bind
28783	4	7307	7	10	NULL	0	NULL	statement 2	NULL		does not inhibit	NULL				cytosolic Ca2+	NULL	mobilization of 			NULL		NULL	NULL	NULL	NULL	gw60_circulation_93_6_1201_s_129	8653842	21  The aggregation response to shear forces generated in a cone and plate viscometer showed that neither the mobilization of cytosolic Ca2+ nor the aggregation response to shear stress was inhibited by blocking the platelet cyclooxygenase and thromboxane A2 production with ASA. 22  These results suggest that the high levels of shear stress (>30 dyne/cm2) may have induced plasma vWF to bind to platelet GPIb and caused an increase in platelet cytosolic Ca2+ and platelet aggregation, both of which are potentiated by the vWF binding to the platelet GPIIb-IIIa complex.	bind
28784	5	7307	7	10	NULL	0	NULL	statement 1			does not inhibit					statement 14					NULL		NULL	NULL	NULL	NULL	gw60_circulation_93_6_1201_s_129	8653842	21  The aggregation response to shear forces generated in a cone and plate viscometer showed that neither the mobilization of cytosolic Ca2+ nor the aggregation response to shear stress was inhibited by blocking the platelet cyclooxygenase and thromboxane A2 production with ASA. 22  These results suggest that the high levels of shear stress (>30 dyne/cm2) may have induced plasma vWF to bind to platelet GPIb and caused an increase in platelet cytosolic Ca2+ and platelet aggregation, both of which are potentiated by the vWF binding to the platelet GPIIb-IIIa complex.	bind
28785	6	7307	7	10	NULL	0	NULL	statement 2			does not inhibit					statement 14					NULL		NULL	NULL	NULL	NULL	gw60_circulation_93_6_1201_s_129	8653842	21  The aggregation response to shear forces generated in a cone and plate viscometer showed that neither the mobilization of cytosolic Ca2+ nor the aggregation response to shear stress was inhibited by blocking the platelet cyclooxygenase and thromboxane A2 production with ASA. 22  These results suggest that the high levels of shear stress (>30 dyne/cm2) may have induced plasma vWF to bind to platelet GPIb and caused an increase in platelet cytosolic Ca2+ and platelet aggregation, both of which are potentiated by the vWF binding to the platelet GPIIb-IIIa complex.	bind
28786	7	7307	7	NULL	NULL	0	NULL	vWF	NULL	plasma	bind	NULL				GPIb	NULL	platelet			NULL		0	NULL	NULL	NULL	gw60_circulation_93_6_1201_s_129	8653842	21  The aggregation response to shear forces generated in a cone and plate viscometer showed that neither the mobilization of cytosolic Ca2+ nor the aggregation response to shear stress was inhibited by blocking the platelet cyclooxygenase and thromboxane A2 production with ASA. 22  These results suggest that the high levels of shear stress (>30 dyne/cm2) may have induced plasma vWF to bind to platelet GPIb and caused an increase in platelet cytosolic Ca2+ and platelet aggregation, both of which are potentiated by the vWF binding to the platelet GPIIb-IIIa complex.	bind
28787	8	7307	7	NULL	NULL	0	NULL	shear stress	NULL	high levels of	induce	NULL	may			statement 7	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_93_6_1201_s_129	8653842	21  The aggregation response to shear forces generated in a cone and plate viscometer showed that neither the mobilization of cytosolic Ca2+ nor the aggregation response to shear stress was inhibited by blocking the platelet cyclooxygenase and thromboxane A2 production with ASA. 22  These results suggest that the high levels of shear stress (>30 dyne/cm2) may have induced plasma vWF to bind to platelet GPIb and caused an increase in platelet cytosolic Ca2+ and platelet aggregation, both of which are potentiated by the vWF binding to the platelet GPIIb-IIIa complex.	bind
28788	9	7307	7	10	NULL	0	NULL	shear stress	NULL	high levels of	increase	NULL				cytosolic Ca2+	NULL	platelet 			NULL		NULL	NULL	NULL	NULL	gw60_circulation_93_6_1201_s_129	8653842	21  The aggregation response to shear forces generated in a cone and plate viscometer showed that neither the mobilization of cytosolic Ca2+ nor the aggregation response to shear stress was inhibited by blocking the platelet cyclooxygenase and thromboxane A2 production with ASA. 22  These results suggest that the high levels of shear stress (>30 dyne/cm2) may have induced plasma vWF to bind to platelet GPIb and caused an increase in platelet cytosolic Ca2+ and platelet aggregation, both of which are potentiated by the vWF binding to the platelet GPIIb-IIIa complex.	bind
28789	10	7307	7	NULL	NULL	0	NULL	shear stress	NULL	high levels of	increase	NULL				platelet aggregation	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_93_6_1201_s_129	8653842	21  The aggregation response to shear forces generated in a cone and plate viscometer showed that neither the mobilization of cytosolic Ca2+ nor the aggregation response to shear stress was inhibited by blocking the platelet cyclooxygenase and thromboxane A2 production with ASA. 22  These results suggest that the high levels of shear stress (>30 dyne/cm2) may have induced plasma vWF to bind to platelet GPIb and caused an increase in platelet cytosolic Ca2+ and platelet aggregation, both of which are potentiated by the vWF binding to the platelet GPIIb-IIIa complex.	bind
28790	11	7307	7	NULL	NULL	0	NULL	vWF	NULL		bind	NULL				GPIIb-IIIa complex	NULL	platelet			NULL		0	NULL	NULL	NULL	gw60_circulation_93_6_1201_s_129	8653842	21  The aggregation response to shear forces generated in a cone and plate viscometer showed that neither the mobilization of cytosolic Ca2+ nor the aggregation response to shear stress was inhibited by blocking the platelet cyclooxygenase and thromboxane A2 production with ASA. 22  These results suggest that the high levels of shear stress (>30 dyne/cm2) may have induced plasma vWF to bind to platelet GPIb and caused an increase in platelet cytosolic Ca2+ and platelet aggregation, both of which are potentiated by the vWF binding to the platelet GPIIb-IIIa complex.	bind
28791	12	7307	7	NULL	NULL	0	NULL	statement 11	NULL		potentiates	NULL				statement 9	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_93_6_1201_s_129	8653842	21  The aggregation response to shear forces generated in a cone and plate viscometer showed that neither the mobilization of cytosolic Ca2+ nor the aggregation response to shear stress was inhibited by blocking the platelet cyclooxygenase and thromboxane A2 production with ASA. 22  These results suggest that the high levels of shear stress (>30 dyne/cm2) may have induced plasma vWF to bind to platelet GPIb and caused an increase in platelet cytosolic Ca2+ and platelet aggregation, both of which are potentiated by the vWF binding to the platelet GPIIb-IIIa complex.	bind
28792	13	7307	7	NULL	NULL	0	NULL	statement 11	NULL		potentiates	NULL				statement 10	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_93_6_1201_s_129	8653842	21  The aggregation response to shear forces generated in a cone and plate viscometer showed that neither the mobilization of cytosolic Ca2+ nor the aggregation response to shear stress was inhibited by blocking the platelet cyclooxygenase and thromboxane A2 production with ASA. 22  These results suggest that the high levels of shear stress (>30 dyne/cm2) may have induced plasma vWF to bind to platelet GPIb and caused an increase in platelet cytosolic Ca2+ and platelet aggregation, both of which are potentiated by the vWF binding to the platelet GPIIb-IIIa complex.	bind
54471	14	7307	7	10	NULL	0	NULL	shear stress			induce					aggregation					NULL		0	NULL	NULL	NULL	gw60_circulation_93_6_1201_s_129	8653842	21  The aggregation response to shear forces generated in a cone and plate viscometer showed that neither the mobilization of cytosolic Ca2+ nor the aggregation response to shear stress was inhibited by blocking the platelet cyclooxygenase and thromboxane A2 production with ASA. 22  These results suggest that the high levels of shear stress (>30 dyne/cm2) may have induced plasma vWF to bind to platelet GPIb and caused an increase in platelet cytosolic Ca2+ and platelet aggregation, both of which are potentiated by the vWF binding to the platelet GPIIb-IIIa complex.	bind
26440	1	7308	5	13	NULL	NULL	NULL	factor VIIa	GP		bind					TF	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_2_409_s_259	9081698	21  The second is the inhibition of factor Xa - catalyzed back activation to VIIa of factor VII molecules bound to TF.	bind
26441	2	7308	5	13	NULL	NULL	NULL	factor Xa	GP	inhibition of	catalyzes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_2_409_s_259	9081698	21  The second is the inhibition of factor Xa - catalyzed back activation to VIIa of factor VII molecules bound to TF.	bind
28793	1	7308	7	NULL	NULL	0	NULL	factor VIIa	NULL		bind	NULL				TF	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_2_409_s_259	9081698	21  The second is the inhibition of factor Xa - catalyzed back activation to VIIa of factor VII molecules bound to TF.	bind
28794	2	7308	7	10	NULL	0	NULL	factor Xa	NULL	inhibition of	catalyzes	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_2_409_s_259	9081698	21  The second is the inhibition of factor Xa - catalyzed back activation to VIIa of factor VII molecules bound to TF.	bind
28795	3	7308	7	NULL	NULL	0	NULL	factor VIIa	NULL		is a type of	NULL				factor VII	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_2_409_s_259	9081698	21  The second is the inhibition of factor Xa - catalyzed back activation to VIIa of factor VII molecules bound to TF.	bind
26442	1	7309	5	13	NULL	NULL	NULL	ECM	CellComponent		bind					TIMP-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_3_296_s_176	10645926	21  Under these circumstances, ECM binding of TIMP-3 may become saturated by overexpression, resulting in the generation of local levels of a soluble form of TIMP-3.	bind
26443	2	7309	5	13	NULL	NULL	NULL	TIMP-3	GP	overexpression of	saturates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_3_296_s_176	10645926	21  Under these circumstances, ECM binding of TIMP-3 may become saturated by overexpression, resulting in the generation of local levels of a soluble form of TIMP-3.	bind
26444	3	7309	5	13	NULL	NULL	NULL	statement 2	Process		generates					TIMP-3	GP	soluble forms of 			NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_3_296_s_176	10645926	21  Under these circumstances, ECM binding of TIMP-3 may become saturated by overexpression, resulting in the generation of local levels of a soluble form of TIMP-3.	bind
28796	1	7309	7	13	NULL	NULL	NULL	ECM	CellComponent		bind					TIMP-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_3_296_s_176	10645926	21  Under these circumstances, ECM binding of TIMP-3 may become saturated by overexpression, resulting in the generation of local levels of a soluble form of TIMP-3.	bind
28797	3	7309	7	10	NULL	0	NULL	statement 2	NULL		generates	NULL				TIMP-3	NULL	soluble form of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_3_296_s_176	10645926	21  Under these circumstances, ECM binding of TIMP-3 may become saturated by overexpression, resulting in the generation of local levels of a soluble form of TIMP-3.	bind
46546	2	7309	7	10	NULL	0	NULL	TIMP-3	NULL	overexpression of	saturates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_101_3_296_s_176	10645926	21  Under these circumstances, ECM binding of TIMP-3 may become saturated by overexpression, resulting in the generation of local levels of a soluble form of TIMP-3.	bind
26445	1	7310	5	13	NULL	NULL	NULL	mAb anti-C3-9	GP		is a type of					capture antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_10_3542_s_82	9396453	21 - 23 Briefly, C3b/c was measured with mAb anti-C3-9 as capture antibody, which binds to C3b, iC3b, C3c, as well as iC3 (C3b-like C3).	bind
26446	2	7310	5	13	NULL	NULL	NULL	mAb anti-C3-9	GP		bind					C3b	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_10_3542_s_82	9396453	21 - 23 Briefly, C3b/c was measured with mAb anti-C3-9 as capture antibody, which binds to C3b, iC3b, C3c, as well as iC3 (C3b-like C3).	bind
26447	3	7310	5	13	NULL	NULL	NULL	mAb anti-C3-9	GP		bind					iC3b	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_10_3542_s_82	9396453	21 - 23 Briefly, C3b/c was measured with mAb anti-C3-9 as capture antibody, which binds to C3b, iC3b, C3c, as well as iC3 (C3b-like C3).	bind
26448	4	7310	5	13	NULL	NULL	NULL	mAb anti-C3-9	GP		bind					C3c	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_10_3542_s_82	9396453	21 - 23 Briefly, C3b/c was measured with mAb anti-C3-9 as capture antibody, which binds to C3b, iC3b, C3c, as well as iC3 (C3b-like C3).	bind
26449	5	7310	5	13	NULL	NULL	NULL	mAb anti-C3-9	GP		bind					iC3	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_10_3542_s_82	9396453	21 - 23 Briefly, C3b/c was measured with mAb anti-C3-9 as capture antibody, which binds to C3b, iC3b, C3c, as well as iC3 (C3b-like C3).	bind
26450	6	7310	5	13	NULL	NULL	NULL	iC3	GP		is					C3b-like C3	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_10_3542_s_82	9396453	21 - 23 Briefly, C3b/c was measured with mAb anti-C3-9 as capture antibody, which binds to C3b, iC3b, C3c, as well as iC3 (C3b-like C3).	bind
28798	1	7310	7	10	NULL	0	NULL	 mAb anti-C3-9			binds to					C3b					NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_10_3542_s_82	9396453	21 - 23 Briefly, C3b/c was measured with mAb anti-C3-9 as capture antibody, which binds to C3b, iC3b, C3c, as well as iC3 (C3b-like C3).	bind
28799	2	7310	7	10	NULL	0	NULL	 mAb anti-C3-9			bind					iC3b					NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_10_3542_s_82	9396453	21 - 23 Briefly, C3b/c was measured with mAb anti-C3-9 as capture antibody, which binds to C3b, iC3b, C3c, as well as iC3 (C3b-like C3).	bind
28800	3	7310	7	10	NULL	0	NULL	mAb anti-C3-9			bind					C3c					NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_10_3542_s_82	9396453	21 - 23 Briefly, C3b/c was measured with mAb anti-C3-9 as capture antibody, which binds to C3b, iC3b, C3c, as well as iC3 (C3b-like C3).	bind
28801	4	7310	7	10	NULL	0	NULL	mAb anti-C3-9			bind					iC3					NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_10_3542_s_82	9396453	21 - 23 Briefly, C3b/c was measured with mAb anti-C3-9 as capture antibody, which binds to C3b, iC3b, C3c, as well as iC3 (C3b-like C3).	bind
28802	5	7310	7	10	NULL	0	NULL	iC3			is					C3b-like C3					NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_10_3542_s_82	9396453	21 - 23 Briefly, C3b/c was measured with mAb anti-C3-9 as capture antibody, which binds to C3b, iC3b, C3c, as well as iC3 (C3b-like C3).	bind
54792	6	7310	7	10	NULL	0	NULL	mAb anti-C3-9			is a type of					capture antibody					NULL		0	NULL	NULL	NULL	gw60_circulation_96_10_3542_s_82	9396453	21 - 23 Briefly, C3b/c was measured with mAb anti-C3-9 as capture antibody, which binds to C3b, iC3b, C3c, as well as iC3 (C3b-like C3).	bind
26451	1	7311	5	13	NULL	NULL	NULL	ATF2 homodimer	GP		recognizes;;binds							specific		ATF/CRE motifs	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_42	16497991	21 Although ATF2 recognizes and binds specific ATF/CRE motifs as a homo- or heterodimer in the same fashion as CREB, the differential role of ATF2 and CREB remains largely uncharacterized.	bind
26453	2	7311	5	13	NULL	NULL	NULL	ATF2 heterodimer	GP		recognizes;;binds							specific		ATF/CRE motifs	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_42	16497991	21 Although ATF2 recognizes and binds specific ATF/CRE motifs as a homo- or heterodimer in the same fashion as CREB, the differential role of ATF2 and CREB remains largely uncharacterized.	bind
26455	3	7311	5	13	NULL	NULL	NULL	CREB homodimer	GP		recognizes;;binds							specific		ATF/CRE motifs	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_42	16497991	21 Although ATF2 recognizes and binds specific ATF/CRE motifs as a homo- or heterodimer in the same fashion as CREB, the differential role of ATF2 and CREB remains largely uncharacterized.	bind
26457	4	7311	5	13	NULL	NULL	NULL	CREB heterodimer	GP		recognizes;;binds							specific		ATF/CRE motifs	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_42	16497991	21 Although ATF2 recognizes and binds specific ATF/CRE motifs as a homo- or heterodimer in the same fashion as CREB, the differential role of ATF2 and CREB remains largely uncharacterized.	bind
26458	5	7311	5	13	NULL	NULL	NULL	statement 3	Process		same manner as					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_42	16497991	21 Although ATF2 recognizes and binds specific ATF/CRE motifs as a homo- or heterodimer in the same fashion as CREB, the differential role of ATF2 and CREB remains largely uncharacterized.	bind
26459	6	7311	5	13	NULL	NULL	NULL	statement 4	Process		same manner as					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_42	16497991	21 Although ATF2 recognizes and binds specific ATF/CRE motifs as a homo- or heterodimer in the same fashion as CREB, the differential role of ATF2 and CREB remains largely uncharacterized.	bind
28803	1	7311	7	NULL	NULL	0	NULL	ATF2 homodimer	NULL		recognizes	NULL					NULL			ATF/CRE motifs 	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_42	16497991	21 Although ATF2 recognizes and binds specific ATF/CRE motifs as a homo- or heterodimer in the same fashion as CREB, the differential role of ATF2 and CREB remains largely uncharacterized.	bind
28804	2	7311	7	NULL	NULL	0	NULL	ATF2 heterodimer	NULL		recognizes	NULL					NULL			ATF/CRE motifs 	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_42	16497991	21 Although ATF2 recognizes and binds specific ATF/CRE motifs as a homo- or heterodimer in the same fashion as CREB, the differential role of ATF2 and CREB remains largely uncharacterized.	bind
28805	6	7311	7	NULL	NULL	0	NULL	statement 1	NULL		same as	NULL				statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_42	16497991	21 Although ATF2 recognizes and binds specific ATF/CRE motifs as a homo- or heterodimer in the same fashion as CREB, the differential role of ATF2 and CREB remains largely uncharacterized.	bind
28806	7	7311	7	NULL	NULL	0	NULL	statement 2	NULL		same as	NULL				statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_42	16497991	21 Although ATF2 recognizes and binds specific ATF/CRE motifs as a homo- or heterodimer in the same fashion as CREB, the differential role of ATF2 and CREB remains largely uncharacterized.	bind
28807	5	7311	7	NULL	NULL	0	NULL	CREB	NULL		bind	NULL					NULL			ATF/CRE motifs 	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_42	16497991	21 Although ATF2 recognizes and binds specific ATF/CRE motifs as a homo- or heterodimer in the same fashion as CREB, the differential role of ATF2 and CREB remains largely uncharacterized.	bind
46597	3	7311	7	NULL	NULL	0	NULL	ATF2 homodimer	NULL		bind	NULL					NULL			 ATF/CRE motifs	NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_42	16497991	21 Although ATF2 recognizes and binds specific ATF/CRE motifs as a homo- or heterodimer in the same fashion as CREB, the differential role of ATF2 and CREB remains largely uncharacterized.	bind
46598	4	7311	7	NULL	NULL	0	NULL	ATF2 heterodimer	NULL		bind	NULL					NULL			ATF/CRE motifs 	NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_42	16497991	21 Although ATF2 recognizes and binds specific ATF/CRE motifs as a homo- or heterodimer in the same fashion as CREB, the differential role of ATF2 and CREB remains largely uncharacterized.	bind
46599	8	7311	7	NULL	NULL	0	NULL	statement 3	NULL		same as	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_42	16497991	21 Although ATF2 recognizes and binds specific ATF/CRE motifs as a homo- or heterodimer in the same fashion as CREB, the differential role of ATF2 and CREB remains largely uncharacterized.	bind
46600	9	7311	7	NULL	NULL	0	NULL	statement 4	NULL		same as	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_42	16497991	21 Although ATF2 recognizes and binds specific ATF/CRE motifs as a homo- or heterodimer in the same fashion as CREB, the differential role of ATF2 and CREB remains largely uncharacterized.	bind
26460	1	7312	5	13	NULL	NULL	NULL	Ras	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_23_2955_s_160	12782568	21 Binding of  Ras to GTP results in the activation of  Raf kinase, which then phosphorylates MEK triggering the sequential phosphorylation of the MAPK module.	bind
26461	2	7312	5	13	NULL	NULL	NULL	statement 1	Process		results in					Raf kinase	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_23_2955_s_160	12782568	21 Binding of  Ras to GTP results in the activation of  Raf kinase, which then phosphorylates MEK triggering the sequential phosphorylation of the MAPK module.	bind
26462	3	7312	5	13	NULL	NULL	NULL	Raf kinase	GP	activated	phosphorylates					MEK	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_23_2955_s_160	12782568	21 Binding of  Ras to GTP results in the activation of  Raf kinase, which then phosphorylates MEK triggering the sequential phosphorylation of the MAPK module.	bind
26463	4	7312	5	13	NULL	NULL	NULL	statement 3	Process		triggers					MAPK module	Process	sequential phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_23_2955_s_160	12782568	21 Binding of  Ras to GTP results in the activation of  Raf kinase, which then phosphorylates MEK triggering the sequential phosphorylation of the MAPK module.	bind
28808	1	7312	7	NULL	NULL	0	NULL	Ras	NULL		binds	NULL				GTP	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_107_23_2955_s_160	12782568	21 Binding of  Ras to GTP results in the activation of  Raf kinase, which then phosphorylates MEK triggering the sequential phosphorylation of the MAPK module.	bind
28809	2	7312	7	NULL	NULL	0	NULL	statement 1	NULL		activates	NULL				Raf kinase	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_107_23_2955_s_160	12782568	21 Binding of  Ras to GTP results in the activation of  Raf kinase, which then phosphorylates MEK triggering the sequential phosphorylation of the MAPK module.	bind
28810	3	7312	7	NULL	NULL	0	NULL	Raf kinase	NULL	activated 	phosphorylates	NULL				MEK	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_107_23_2955_s_160	12782568	21 Binding of  Ras to GTP results in the activation of  Raf kinase, which then phosphorylates MEK triggering the sequential phosphorylation of the MAPK module.	bind
28811	4	7312	7	NULL	NULL	0	NULL	statement 3	NULL		triggers	NULL				MAPK module	NULL	 sequential phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_circulation_107_23_2955_s_160	12782568	21 Binding of  Ras to GTP results in the activation of  Raf kinase, which then phosphorylates MEK triggering the sequential phosphorylation of the MAPK module.	bind
26464	1	7313	5	13	NULL	NULL	NULL	lipoprotein	GP		interacts with					APG	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2507_s_29	9409221	21 It is predictable that such therapy affects lipoprotein-APG interaction, and it has recently been shown that drugs can reduce total LDL binding with APG.	bind
26465	2	7313	5	13	NULL	NULL	NULL	LDL	GP		bind					APG	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2507_s_29	9409221	21 It is predictable that such therapy affects lipoprotein-APG interaction, and it has recently been shown that drugs can reduce total LDL binding with APG.	bind
26466	3	7313	5	13	NULL	NULL	NULL	drugs	Chemical		reduces					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2507_s_29	9409221	21 It is predictable that such therapy affects lipoprotein-APG interaction, and it has recently been shown that drugs can reduce total LDL binding with APG.	bind
28812	1	7313	7	NULL	NULL	0	NULL	lipoprotein	NULL		interacts with	NULL				APG	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2507_s_29	9409221	21 It is predictable that such therapy affects lipoprotein-APG interaction, and it has recently been shown that drugs can reduce total LDL binding with APG.	bind
28813	2	7313	7	NULL	NULL	0	NULL	total LDL	NULL		bind	NULL				APG	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2507_s_29	9409221	21 It is predictable that such therapy affects lipoprotein-APG interaction, and it has recently been shown that drugs can reduce total LDL binding with APG.	bind
28814	3	7313	7	NULL	NULL	0	NULL	drugs	NULL		reduce	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2507_s_29	9409221	21 It is predictable that such therapy affects lipoprotein-APG interaction, and it has recently been shown that drugs can reduce total LDL binding with APG.	bind
26467	1	7314	5	13	NULL	NULL	NULL	TRL particles	GP		bind					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1470_s_105	12231568	21 More specifically, apoC-I inhibits apoE-mediated binding of TRL particles to the LDL receptor and to the LDL receptor-like protein.	bind
26468	2	7314	5	13	NULL	NULL	NULL	apoE	GP		mediates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1470_s_105	12231568	21 More specifically, apoC-I inhibits apoE-mediated binding of TRL particles to the LDL receptor and to the LDL receptor-like protein.	bind
26469	3	7314	5	13	NULL	NULL	NULL	apoC-I	GP		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1470_s_105	12231568	21 More specifically, apoC-I inhibits apoE-mediated binding of TRL particles to the LDL receptor and to the LDL receptor-like protein.	bind
26470	4	7314	5	13	NULL	NULL	NULL	TRL particles	GP		bind					LDL receptor-like protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1470_s_105	12231568	21 More specifically, apoC-I inhibits apoE-mediated binding of TRL particles to the LDL receptor and to the LDL receptor-like protein.	bind
26471	5	7314	5	13	NULL	NULL	NULL	apoE	GP		mediates					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1470_s_105	12231568	21 More specifically, apoC-I inhibits apoE-mediated binding of TRL particles to the LDL receptor and to the LDL receptor-like protein.	bind
26472	6	7314	5	13	NULL	NULL	NULL	apoC-I	GP		inhibit					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1470_s_105	12231568	21 More specifically, apoC-I inhibits apoE-mediated binding of TRL particles to the LDL receptor and to the LDL receptor-like protein.	bind
28815	1	7314	7	NULL	NULL	0	NULL	TRL particles	NULL		bind	NULL				LDL receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1470_s_105	12231568	21 More specifically, apoC-I inhibits apoE-mediated binding of TRL particles to the LDL receptor and to the LDL receptor-like protein.	bind
28816	2	7314	7	NULL	NULL	0	NULL	TRL particles	NULL		bind	NULL				LDL receptor-like protein	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1470_s_105	12231568	21 More specifically, apoC-I inhibits apoE-mediated binding of TRL particles to the LDL receptor and to the LDL receptor-like protein.	bind
28817	3	7314	7	NULL	NULL	0	NULL	apoE	NULL		mediates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1470_s_105	12231568	21 More specifically, apoC-I inhibits apoE-mediated binding of TRL particles to the LDL receptor and to the LDL receptor-like protein.	bind
28818	4	7314	7	NULL	NULL	0	NULL	apoE	NULL		mediates	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1470_s_105	12231568	21 More specifically, apoC-I inhibits apoE-mediated binding of TRL particles to the LDL receptor and to the LDL receptor-like protein.	bind
28819	5	7314	7	NULL	NULL	0	NULL	apoC-I 	NULL		inhibits	NULL	specifically			statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1470_s_105	12231568	21 More specifically, apoC-I inhibits apoE-mediated binding of TRL particles to the LDL receptor and to the LDL receptor-like protein.	bind
28820	6	7314	7	NULL	NULL	0	NULL	apoC-I 	NULL		inhibits	NULL	specifically			statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1470_s_105	12231568	21 More specifically, apoC-I inhibits apoE-mediated binding of TRL particles to the LDL receptor and to the LDL receptor-like protein.	bind
26473	1	7315	5	13	NULL	NULL	NULL	PPAR-alpha	GP	activated	bind					AP-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_109_7_904_s_172	14967736	21 Therefore, it is considered that activated PPAR-alpha binds to AP-1 or its cofactor and that AP-1 is prevented from binding to the cis-elements of the promoter region, which results in impairment of ET-1 gene induction.	bind
26474	2	7315	5	13	NULL	NULL	NULL	PPAR-alpha	GP	activated	bind					AP-1 cofactor	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_109_7_904_s_172	14967736	21 Therefore, it is considered that activated PPAR-alpha binds to AP-1 or its cofactor and that AP-1 is prevented from binding to the cis-elements of the promoter region, which results in impairment of ET-1 gene induction.	bind
26475	3	7315	5	13	NULL	NULL	NULL	AP-1	GP		bind									cis-elements of promoter region	NULL		NULL	NULL	NULL	NULL	gw70_circulation_109_7_904_s_172	14967736	21 Therefore, it is considered that activated PPAR-alpha binds to AP-1 or its cofactor and that AP-1 is prevented from binding to the cis-elements of the promoter region, which results in impairment of ET-1 gene induction.	bind
26476	4	7315	5	13	NULL	NULL	NULL	statement 1	Process		prevents					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_109_7_904_s_172	14967736	21 Therefore, it is considered that activated PPAR-alpha binds to AP-1 or its cofactor and that AP-1 is prevented from binding to the cis-elements of the promoter region, which results in impairment of ET-1 gene induction.	bind
54472	5	7315	5	13	NULL	NULL	NULL	statement 2	Process		prevents					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_109_7_904_s_172	14967736	21 Therefore, it is considered that activated PPAR-alpha binds to AP-1 or its cofactor and that AP-1 is prevented from binding to the cis-elements of the promoter region, which results in impairment of ET-1 gene induction.	bind
54473	7	7315	5	13	NULL	NULL	NULL	statement 4	Process		impairs					ET-1 gene	GP	induction of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_109_7_904_s_172	14967736	21 Therefore, it is considered that activated PPAR-alpha binds to AP-1 or its cofactor and that AP-1 is prevented from binding to the cis-elements of the promoter region, which results in impairment of ET-1 gene induction.	bind
54474	8	7315	5	13	NULL	NULL	NULL	statement 5	Process		impairs					ET-1 gene	GP	induction of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_109_7_904_s_172	14967736	21 Therefore, it is considered that activated PPAR-alpha binds to AP-1 or its cofactor and that AP-1 is prevented from binding to the cis-elements of the promoter region, which results in impairment of ET-1 gene induction.	bind
28821	1	7315	7	NULL	NULL	0	NULL	PPAR-alpha	NULL	activated	binds to	NULL				AP-1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_109_7_904_s_172	14967736	21 Therefore, it is considered that activated PPAR-alpha binds to AP-1 or its cofactor and that AP-1 is prevented from binding to the cis-elements of the promoter region, which results in impairment of ET-1 gene induction.	bind
28822	2	7315	7	NULL	NULL	0	NULL	PPAR-alpha	NULL	activated	binds	NULL				AP-1 cofactor	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_109_7_904_s_172	14967736	21 Therefore, it is considered that activated PPAR-alpha binds to AP-1 or its cofactor and that AP-1 is prevented from binding to the cis-elements of the promoter region, which results in impairment of ET-1 gene induction.	bind
28823	3	7315	7	NULL	NULL	0	NULL	AP-1	NULL		bind	NULL					NULL	cis-elements of the promoter			NULL		0	NULL	NULL	NULL	gw70_circulation_109_7_904_s_172	14967736	21 Therefore, it is considered that activated PPAR-alpha binds to AP-1 or its cofactor and that AP-1 is prevented from binding to the cis-elements of the promoter region, which results in impairment of ET-1 gene induction.	bind
28824	4	7315	7	NULL	NULL	0	NULL	statement 1	NULL		prevents	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_109_7_904_s_172	14967736	21 Therefore, it is considered that activated PPAR-alpha binds to AP-1 or its cofactor and that AP-1 is prevented from binding to the cis-elements of the promoter region, which results in impairment of ET-1 gene induction.	bind
28825	5	7315	7	NULL	NULL	0	NULL	statement 2	NULL		prevents	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_109_7_904_s_172	14967736	21 Therefore, it is considered that activated PPAR-alpha binds to AP-1 or its cofactor and that AP-1 is prevented from binding to the cis-elements of the promoter region, which results in impairment of ET-1 gene induction.	bind
28826	6	7315	7	NULL	NULL	0	NULL	statement 4	NULL		impairs	NULL				ET-1 gene	NULL	induction of			NULL		0	NULL	NULL	NULL	gw70_circulation_109_7_904_s_172	14967736	21 Therefore, it is considered that activated PPAR-alpha binds to AP-1 or its cofactor and that AP-1 is prevented from binding to the cis-elements of the promoter region, which results in impairment of ET-1 gene induction.	bind
28827	7	7315	7	NULL	NULL	0	NULL	statement 5	NULL		impairs	NULL				ET-1 gene	NULL	induction of			NULL		0	NULL	NULL	NULL	gw70_circulation_109_7_904_s_172	14967736	21 Therefore, it is considered that activated PPAR-alpha binds to AP-1 or its cofactor and that AP-1 is prevented from binding to the cis-elements of the promoter region, which results in impairment of ET-1 gene induction.	bind
26477	1	7316	5	13	NULL	NULL	NULL	Cdk inhibitors	GP		regulates					Cyclin-Cdk	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_5_1511_s_27	10550307	21, 22 Cyclin-Cdk activity is, in turn, regulated by Cdk inhibitors, which bind the Cdk-cyclin complexes, inhibit their activity, and block cell cycle progression.	bind
26478	2	7316	5	13	NULL	NULL	NULL	Cdk inhibitors	GP		bind					Cdk-cyclin complexes	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_5_1511_s_27	10550307	21, 22 Cyclin-Cdk activity is, in turn, regulated by Cdk inhibitors, which bind the Cdk-cyclin complexes, inhibit their activity, and block cell cycle progression.	bind
26479	3	7316	5	13	NULL	NULL	NULL	statement 2	Process		inhibit					Cdk-cyclin complexes	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_5_1511_s_27	10550307	21, 22 Cyclin-Cdk activity is, in turn, regulated by Cdk inhibitors, which bind the Cdk-cyclin complexes, inhibit their activity, and block cell cycle progression.	bind
26480	4	7316	5	13	NULL	NULL	NULL	statement 3	Process		blocks					cell cycle progression	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_5_1511_s_27	10550307	21, 22 Cyclin-Cdk activity is, in turn, regulated by Cdk inhibitors, which bind the Cdk-cyclin complexes, inhibit their activity, and block cell cycle progression.	bind
29086	1	7316	7	NULL	NULL	0	NULL	Cdk inhibitors	NULL		regulate	NULL				Cyclin-Cdk	NULL	activity of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_5_1511_s_27	10550307	21, 22 Cyclin-Cdk activity is, in turn, regulated by Cdk inhibitors, which bind the Cdk-cyclin complexes, inhibit their activity, and block cell cycle progression.	bind
29087	2	7316	7	NULL	NULL	0	NULL	Cdk inhibitors	NULL		bind	NULL				Cdk-cyclin complexes	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_5_1511_s_27	10550307	21, 22 Cyclin-Cdk activity is, in turn, regulated by Cdk inhibitors, which bind the Cdk-cyclin complexes, inhibit their activity, and block cell cycle progression.	bind
29088	3	7316	7	NULL	NULL	0	NULL	statement 2	NULL		inhibit 	NULL				Cdk-cyclin complexes	NULL	activity of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_5_1511_s_27	10550307	21, 22 Cyclin-Cdk activity is, in turn, regulated by Cdk inhibitors, which bind the Cdk-cyclin complexes, inhibit their activity, and block cell cycle progression.	bind
29089	4	7316	7	NULL	NULL	0	NULL	statement 3	NULL		block	NULL				cell cycle progression	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_5_1511_s_27	10550307	21, 22 Cyclin-Cdk activity is, in turn, regulated by Cdk inhibitors, which bind the Cdk-cyclin complexes, inhibit their activity, and block cell cycle progression.	bind
26481	1	7317	5	13	NULL	NULL	NULL	Hdm2	GP		bind					p53	GP				NULL	in HL tissue samples	NULL	NULL	NULL	NULL	gw60_amjpathol_160_2_569_s_199	11839577	21, 29  The observations from this study of HL tissue samples and cell lines show that, in parallel with the absence of these Hdm2/p14ARF complexes, p53 is bound by Hdm2, which under different circumstances has been shown to inactivate the ability of p53 to induce the expression of p53-transactivated genes.	bind
26482	2	7317	5	13	NULL	NULL	NULL	p53 	GP		induces					p53-transactivated genes	Process	expression of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_2_569_s_199	11839577	21, 29  The observations from this study of HL tissue samples and cell lines show that, in parallel with the absence of these Hdm2/p14ARF complexes, p53 is bound by Hdm2, which under different circumstances has been shown to inactivate the ability of p53 to induce the expression of p53-transactivated genes.	bind
26483	3	7317	5	13	NULL	NULL	NULL	statement 1	Process		inactivates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_2_569_s_199	11839577	21, 29  The observations from this study of HL tissue samples and cell lines show that, in parallel with the absence of these Hdm2/p14ARF complexes, p53 is bound by Hdm2, which under different circumstances has been shown to inactivate the ability of p53 to induce the expression of p53-transactivated genes.	bind
29090	1	7317	7	NULL	NULL	0	NULL	Hdm2	NULL		bind	NULL				p53	NULL				NULL	HL tissue samples	0	NULL	NULL	NULL	gw60_amjpathol_160_2_569_s_199	11839577	21, 29  The observations from this study of HL tissue samples and cell lines show that, in parallel with the absence of these Hdm2/p14ARF complexes, p53 is bound by Hdm2, which under different circumstances has been shown to inactivate the ability of p53 to induce the expression of p53-transactivated genes.	bind
29091	2	7317	7	NULL	NULL	0	NULL	statement 1	NULL		in absence of	NULL				Hdm2/p14ARF complexes	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_2_569_s_199	11839577	21, 29  The observations from this study of HL tissue samples and cell lines show that, in parallel with the absence of these Hdm2/p14ARF complexes, p53 is bound by Hdm2, which under different circumstances has been shown to inactivate the ability of p53 to induce the expression of p53-transactivated genes.	bind
29092	3	7317	7	NULL	NULL	0	NULL	p53	NULL		induce	NULL				p53-transactivated genes	NULL	expression of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_2_569_s_199	11839577	21, 29  The observations from this study of HL tissue samples and cell lines show that, in parallel with the absence of these Hdm2/p14ARF complexes, p53 is bound by Hdm2, which under different circumstances has been shown to inactivate the ability of p53 to induce the expression of p53-transactivated genes.	bind
29093	4	7317	7	NULL	NULL	0	NULL	Hdm2	NULL		inactivate	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_2_569_s_199	11839577	21, 29  The observations from this study of HL tissue samples and cell lines show that, in parallel with the absence of these Hdm2/p14ARF complexes, p53 is bound by Hdm2, which under different circumstances has been shown to inactivate the ability of p53 to induce the expression of p53-transactivated genes.	bind
26640	1	7318	5	13	NULL	NULL	NULL	HuR	GP		is a type of					ubiquitous mRNA binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_11_1034_s_209	14645134	21,24,81,86,87,140      Stability of sGC-alpha1 mRNA is regulated by the ubiquitous mRNA binding protein HuR, which binds to AU-rich elements in the 3''-untranslated region (UTR) and increases mRNA half-life; cGMP-elevating agents decrease expression and RNA binding of HuR, thereby destabilizing sGC-alpha1 mRNA.	bind
26641	2	7318	5	13	NULL	NULL	NULL	sGC-alpha1 mRNA	NucleicAcid	stability of	is regulated by					HuR	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_11_1034_s_209	14645134	21,24,81,86,87,140      Stability of sGC-alpha1 mRNA is regulated by the ubiquitous mRNA binding protein HuR, which binds to AU-rich elements in the 3''-untranslated region (UTR) and increases mRNA half-life; cGMP-elevating agents decrease expression and RNA binding of HuR, thereby destabilizing sGC-alpha1 mRNA.	bind
26642	3	7318	5	13	NULL	NULL	NULL	HuR	GP		bind									AU-rich elements in 3''-untranslated region	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_11_1034_s_209	14645134	21,24,81,86,87,140      Stability of sGC-alpha1 mRNA is regulated by the ubiquitous mRNA binding protein HuR, which binds to AU-rich elements in the 3''-untranslated region (UTR) and increases mRNA half-life; cGMP-elevating agents decrease expression and RNA binding of HuR, thereby destabilizing sGC-alpha1 mRNA.	bind
26643	4	7318	5	13	NULL	NULL	NULL	statement 3	Process		increases					mRNA	NucleicAcid	half life of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_11_1034_s_209	14645134	21,24,81,86,87,140      Stability of sGC-alpha1 mRNA is regulated by the ubiquitous mRNA binding protein HuR, which binds to AU-rich elements in the 3''-untranslated region (UTR) and increases mRNA half-life; cGMP-elevating agents decrease expression and RNA binding of HuR, thereby destabilizing sGC-alpha1 mRNA.	bind
26644	5	7318	5	13	NULL	NULL	NULL	cGMP-elevating agents	Chemical		decreases					HuR	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_11_1034_s_209	14645134	21,24,81,86,87,140      Stability of sGC-alpha1 mRNA is regulated by the ubiquitous mRNA binding protein HuR, which binds to AU-rich elements in the 3''-untranslated region (UTR) and increases mRNA half-life; cGMP-elevating agents decrease expression and RNA binding of HuR, thereby destabilizing sGC-alpha1 mRNA.	bind
26645	6	7318	5	13	NULL	NULL	NULL	HuR	GP		bind					RNA	NucleicAcid	RNA binding of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_11_1034_s_209	14645134	21,24,81,86,87,140      Stability of sGC-alpha1 mRNA is regulated by the ubiquitous mRNA binding protein HuR, which binds to AU-rich elements in the 3''-untranslated region (UTR) and increases mRNA half-life; cGMP-elevating agents decrease expression and RNA binding of HuR, thereby destabilizing sGC-alpha1 mRNA.	bind
26647	7	7318	5	13	NULL	NULL	NULL	statement 5	Process		destabilizes					sGC-alpha1 mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_11_1034_s_209	14645134	21,24,81,86,87,140      Stability of sGC-alpha1 mRNA is regulated by the ubiquitous mRNA binding protein HuR, which binds to AU-rich elements in the 3''-untranslated region (UTR) and increases mRNA half-life; cGMP-elevating agents decrease expression and RNA binding of HuR, thereby destabilizing sGC-alpha1 mRNA.	bind
26648	8	7318	5	13	NULL	NULL	NULL	statement 6	Process		destabilizes					sGC-alpha1 mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_11_1034_s_209	14645134	21,24,81,86,87,140      Stability of sGC-alpha1 mRNA is regulated by the ubiquitous mRNA binding protein HuR, which binds to AU-rich elements in the 3''-untranslated region (UTR) and increases mRNA half-life; cGMP-elevating agents decrease expression and RNA binding of HuR, thereby destabilizing sGC-alpha1 mRNA.	bind
46554	9	7318	5	13	NULL	NULL	NULL	cGMP-elevating agents	Chemical		decreases					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_11_1034_s_209	14645134	21,24,81,86,87,140      Stability of sGC-alpha1 mRNA is regulated by the ubiquitous mRNA binding protein HuR, which binds to AU-rich elements in the 3''-untranslated region (UTR) and increases mRNA half-life; cGMP-elevating agents decrease expression and RNA binding of HuR, thereby destabilizing sGC-alpha1 mRNA.	bind
29094	1	7318	7	NULL	NULL	0	NULL	HuR	NULL		regulates	NULL				sGC-alpha1 mRNA	NULL	 stability of			NULL		0	NULL	NULL	NULL	gw70_circulationres_93_11_1034_s_209	14645134	21,24,81,86,87,140      Stability of sGC-alpha1 mRNA is regulated by the ubiquitous mRNA binding protein HuR, which binds to AU-rich elements in the 3''-untranslated region (UTR) and increases mRNA half-life; cGMP-elevating agents decrease expression and RNA binding of HuR, thereby destabilizing sGC-alpha1 mRNA.	bind
29095	2	7318	7	10	NULL	0	NULL	HuR			is a type of					ubiquitous mRNA binding protein					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_11_1034_s_209	14645134	21,24,81,86,87,140      Stability of sGC-alpha1 mRNA is regulated by the ubiquitous mRNA binding protein HuR, which binds to AU-rich elements in the 3''-untranslated region (UTR) and increases mRNA half-life; cGMP-elevating agents decrease expression and RNA binding of HuR, thereby destabilizing sGC-alpha1 mRNA.	bind
29096	3	7318	7	10	NULL	0	NULL	HuR	NULL		binds	NULL					NULL			AU-rich elements in 3'' UTR	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_11_1034_s_209	14645134	21,24,81,86,87,140      Stability of sGC-alpha1 mRNA is regulated by the ubiquitous mRNA binding protein HuR, which binds to AU-rich elements in the 3''-untranslated region (UTR) and increases mRNA half-life; cGMP-elevating agents decrease expression and RNA binding of HuR, thereby destabilizing sGC-alpha1 mRNA.	bind
29097	4	7318	7	NULL	NULL	0	NULL	statement 3	NULL		increases	NULL				mRNA 	NULL	half-life of 			NULL		0	NULL	NULL	NULL	gw70_circulationres_93_11_1034_s_209	14645134	21,24,81,86,87,140      Stability of sGC-alpha1 mRNA is regulated by the ubiquitous mRNA binding protein HuR, which binds to AU-rich elements in the 3''-untranslated region (UTR) and increases mRNA half-life; cGMP-elevating agents decrease expression and RNA binding of HuR, thereby destabilizing sGC-alpha1 mRNA.	bind
29098	5	7318	7	NULL	NULL	0	NULL	HuR	NULL		bind	NULL				RNA	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_93_11_1034_s_209	14645134	21,24,81,86,87,140      Stability of sGC-alpha1 mRNA is regulated by the ubiquitous mRNA binding protein HuR, which binds to AU-rich elements in the 3''-untranslated region (UTR) and increases mRNA half-life; cGMP-elevating agents decrease expression and RNA binding of HuR, thereby destabilizing sGC-alpha1 mRNA.	bind
29099	6	7318	7	NULL	NULL	0	NULL	cGMP-elevating agents	NULL		decrease	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_93_11_1034_s_209	14645134	21,24,81,86,87,140      Stability of sGC-alpha1 mRNA is regulated by the ubiquitous mRNA binding protein HuR, which binds to AU-rich elements in the 3''-untranslated region (UTR) and increases mRNA half-life; cGMP-elevating agents decrease expression and RNA binding of HuR, thereby destabilizing sGC-alpha1 mRNA.	bind
29100	7	7318	7	NULL	NULL	0	NULL	cGMP-elevating agents	NULL		decrease	NULL				RNA	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_circulationres_93_11_1034_s_209	14645134	21,24,81,86,87,140      Stability of sGC-alpha1 mRNA is regulated by the ubiquitous mRNA binding protein HuR, which binds to AU-rich elements in the 3''-untranslated region (UTR) and increases mRNA half-life; cGMP-elevating agents decrease expression and RNA binding of HuR, thereby destabilizing sGC-alpha1 mRNA.	bind
29101	8	7318	7	NULL	NULL	0	NULL	statement 6	NULL		destabilize	NULL				sGC-alpha1 mRNA	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_93_11_1034_s_209	14645134	21,24,81,86,87,140      Stability of sGC-alpha1 mRNA is regulated by the ubiquitous mRNA binding protein HuR, which binds to AU-rich elements in the 3''-untranslated region (UTR) and increases mRNA half-life; cGMP-elevating agents decrease expression and RNA binding of HuR, thereby destabilizing sGC-alpha1 mRNA.	bind
29102	9	7318	7	NULL	NULL	0	NULL	statement 7	NULL		destabilize	NULL				sGC-alpha1 mRNA	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_93_11_1034_s_209	14645134	21,24,81,86,87,140      Stability of sGC-alpha1 mRNA is regulated by the ubiquitous mRNA binding protein HuR, which binds to AU-rich elements in the 3''-untranslated region (UTR) and increases mRNA half-life; cGMP-elevating agents decrease expression and RNA binding of HuR, thereby destabilizing sGC-alpha1 mRNA.	bind
26484	1	7319	5	13	NULL	NULL	NULL	ribosomal protein L5	GP	xenopus	bind					5S rRNA	NucleicAcid	oocyte			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2510_s_296	11410658	22       Scripture,J.B. and Huber,P.W. (1996) Analysis of the binding of  Xenopus ribosomal protein L5 to oocyte 5S rRNA.	bind
29103	1	7319	7	NULL	NULL	0	NULL	ribosomal protein L5	NULL	Xenopus	bind	NULL				5S rRNA	NULL	oocyte			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2510_s_296	11410658	22       Scripture,J.B. and Huber,P.W. (1996) Analysis of the binding of  Xenopus ribosomal protein L5 to oocyte 5S rRNA.	bind
26649	1	7320	5	13	NULL	NULL	NULL	LDL particles	GP		bind		abnormally			LDL receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_4_517_s_133	8624773	22  23  Second, our investigations have shown that patients having LDL particles that bind abnormally to LDL receptors and are slowly removed exhibit LDL particles that are enriched with cholesterol.	bind
26651	2	7320	5	13	NULL	NULL	NULL	LDL particles	GP		is enriched with					cholesterol	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_4_517_s_133	8624773	22  23  Second, our investigations have shown that patients having LDL particles that bind abnormally to LDL receptors and are slowly removed exhibit LDL particles that are enriched with cholesterol.	bind
26652	3	7320	5	13	NULL	NULL	NULL	statement 1	Process		exhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_4_517_s_133	8624773	22  23  Second, our investigations have shown that patients having LDL particles that bind abnormally to LDL receptors and are slowly removed exhibit LDL particles that are enriched with cholesterol.	bind
29104	1	7320	7	NULL	NULL	0	NULL	LDL particles	NULL		bind	NULL	abnormally			LDL receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_4_517_s_133	8624773	22  23  Second, our investigations have shown that patients having LDL particles that bind abnormally to LDL receptors and are slowly removed exhibit LDL particles that are enriched with cholesterol.	bind
29105	2	7320	7	10	NULL	0	NULL	LDL particles	NULL		are enriched with	NULL				cholesterol	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_4_517_s_133	8624773	22  23  Second, our investigations have shown that patients having LDL particles that bind abnormally to LDL receptors and are slowly removed exhibit LDL particles that are enriched with cholesterol.	bind
46555	3	7320	7	10	NULL	0	NULL	statement 1	NULL		exhibits	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_4_517_s_133	8624773	22  23  Second, our investigations have shown that patients having LDL particles that bind abnormally to LDL receptors and are slowly removed exhibit LDL particles that are enriched with cholesterol.	bind
26653	1	7325	5	13	NULL	NULL	NULL	LPL	GP		induces					TNFalpha	GP	production of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_6_1405_s_157	10364070	22  Our results, which show that heparinase treatment of human monocytes totally inhibits LPL-induced TNFalpha production, demonstrate that LPL binding to the monocytic cell surface HSPG is required for its effect on TNFalpha production.	bind
26654	2	7325	5	13	NULL	NULL	NULL	heparinase	GP	treatment	inhibit		totally			statement 1	Process				NULL	human monocytes	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_6_1405_s_157	10364070	22  Our results, which show that heparinase treatment of human monocytes totally inhibits LPL-induced TNFalpha production, demonstrate that LPL binding to the monocytic cell surface HSPG is required for its effect on TNFalpha production.	bind
26655	3	7325	5	13	NULL	NULL	NULL	LPL	GP		bind					HSPG	GP	monocytic cell surface 			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_6_1405_s_157	10364070	22  Our results, which show that heparinase treatment of human monocytes totally inhibits LPL-induced TNFalpha production, demonstrate that LPL binding to the monocytic cell surface HSPG is required for its effect on TNFalpha production.	bind
26656	4	7325	5	13	NULL	NULL	NULL	statement 3	Process		is required for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_6_1405_s_157	10364070	22  Our results, which show that heparinase treatment of human monocytes totally inhibits LPL-induced TNFalpha production, demonstrate that LPL binding to the monocytic cell surface HSPG is required for its effect on TNFalpha production.	bind
29106	1	7325	7	NULL	NULL	0	NULL	LPL	NULL		induce	NULL				TNFalpha	NULL	production of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_6_1405_s_157	10364070	22  Our results, which show that heparinase treatment of human monocytes totally inhibits LPL-induced TNFalpha production, demonstrate that LPL binding to the monocytic cell surface HSPG is required for its effect on TNFalpha production.	bind
29107	2	7325	7	10	NULL	0	NULL	heparinise		treatment	inhibit		totally			statement 1					NULL	human monocytes	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_6_1405_s_157	10364070	22  Our results, which show that heparinase treatment of human monocytes totally inhibits LPL-induced TNFalpha production, demonstrate that LPL binding to the monocytic cell surface HSPG is required for its effect on TNFalpha production.	bind
29108	3	7325	7	NULL	NULL	0	NULL	LPL	NULL		bind	NULL				HSPG	NULL	monocytic cell surface			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_6_1405_s_157	10364070	22  Our results, which show that heparinase treatment of human monocytes totally inhibits LPL-induced TNFalpha production, demonstrate that LPL binding to the monocytic cell surface HSPG is required for its effect on TNFalpha production.	bind
29109	4	7325	7	NULL	NULL	0	NULL	statement 3	NULL		is required for	NULL				TNFalpha	NULL	production of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_6_1405_s_157	10364070	22  Our results, which show that heparinase treatment of human monocytes totally inhibits LPL-induced TNFalpha production, demonstrate that LPL binding to the monocytic cell surface HSPG is required for its effect on TNFalpha production.	bind
26657	1	7326	5	13	NULL	NULL	NULL			wt	bind			kringle IV-10		PM-fibrinogen	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_3_392_s_197	8630665	22  Our work now shows that the individual wt kringle IV-10 also binds to PM-fibrinogen via two components, one LBS mediated and another LBS independent.	bind
26659	2	7326	5	13	NULL	NULL	NULL	statement 1	Process		is mediated by								LBS		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_3_392_s_197	8630665	22  Our work now shows that the individual wt kringle IV-10 also binds to PM-fibrinogen via two components, one LBS mediated and another LBS independent.	bind
26660	3	7326	5	13	NULL	NULL	NULL	statement 1	Process		is independent of								LBS		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_3_392_s_197	8630665	22  Our work now shows that the individual wt kringle IV-10 also binds to PM-fibrinogen via two components, one LBS mediated and another LBS independent.	bind
29110	1	7326	7	10	NULL	0	NULL		NULL	wt	binds to	NULL		kringle IV-10		PM-fibrinogen	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_3_392_s_197	8630665	22  Our work now shows that the individual wt kringle IV-10 also binds to PM-fibrinogen via two components, one LBS mediated and another LBS independent.	bind
29111	2	7326	7	10	NULL	0	NULL				mediates			LBS		statement 1					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_3_392_s_197	8630665	22  Our work now shows that the individual wt kringle IV-10 also binds to PM-fibrinogen via two components, one LBS mediated and another LBS independent.	bind
29112	3	7326	7	10	NULL	0	NULL	statement 1			independent of								LBS		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_3_392_s_197	8630665	22  Our work now shows that the individual wt kringle IV-10 also binds to PM-fibrinogen via two components, one LBS mediated and another LBS independent.	bind
26666	1	7328	5	13	NULL	NULL	NULL	growth factors	GP		bind					tyrosine kinase receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1157_s_235	9777947	22  The results of our experiments therefore indicate that stimulation of U-373 MG glioblastoma cells by various growth factors binding to tyrosine kinase receptors leads to a less differentiated phenotype.	bind
26667	2	7328	5	13	NULL	NULL	NULL	statement 1	Process		stimulates					U-373 MG	Cell				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1157_s_235	9777947	22  The results of our experiments therefore indicate that stimulation of U-373 MG glioblastoma cells by various growth factors binding to tyrosine kinase receptors leads to a less differentiated phenotype.	bind
26668	3	7328	5	13	NULL	NULL	NULL	statement 2	Process		leads to					phenotype	Cell	less differentiated			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1157_s_235	9777947	22  The results of our experiments therefore indicate that stimulation of U-373 MG glioblastoma cells by various growth factors binding to tyrosine kinase receptors leads to a less differentiated phenotype.	bind
54475	4	7328	5	13	NULL	NULL	NULL	U-373 MG 	Cell		is a type of					glioblastoma cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1157_s_235	9777947	22  The results of our experiments therefore indicate that stimulation of U-373 MG glioblastoma cells by various growth factors binding to tyrosine kinase receptors leads to a less differentiated phenotype.	bind
29114	1	7328	7	NULL	NULL	0	NULL	growth factors 	NULL		binds to	NULL				tyrosine kinase receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_4_1157_s_235	9777947	22  The results of our experiments therefore indicate that stimulation of U-373 MG glioblastoma cells by various growth factors binding to tyrosine kinase receptors leads to a less differentiated phenotype.	bind
29115	2	7328	7	10	NULL	0	NULL	growth factors			stimulate					U-373 MG					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1157_s_235	9777947	22  The results of our experiments therefore indicate that stimulation of U-373 MG glioblastoma cells by various growth factors binding to tyrosine kinase receptors leads to a less differentiated phenotype.	bind
29116	3	7328	7	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				phenotype	NULL	less differentiated			NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_4_1157_s_235	9777947	22  The results of our experiments therefore indicate that stimulation of U-373 MG glioblastoma cells by various growth factors binding to tyrosine kinase receptors leads to a less differentiated phenotype.	bind
54476	4	7328	7	10	NULL	0	NULL	U-373 MG			is a type of					glioblastoma cells					NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_4_1157_s_235	9777947	22  The results of our experiments therefore indicate that stimulation of U-373 MG glioblastoma cells by various growth factors binding to tyrosine kinase receptors leads to a less differentiated phenotype.	bind
26670	1	7329	5	13	NULL	NULL	NULL	warfarin	Chemical		inhibit					mesangial cell 	warfarin	proliferation of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_4_1423_s_17	11290560	22  These two inhibitors exert their activities in different ways; warfarin inhibits mesangial cell proliferation possibly by inhibiting gamma-carboxylation of Gas6, whereas Axl-Fc blocks the binding of Gas6 to the cell surface Axl by scavenging Gas6.	bind
26672	2	7329	5	13	NULL	NULL	NULL	warfarin	Chemical		inhibit					Gas6	GP	carboxylation of	gamma		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_4_1423_s_17	11290560	22  These two inhibitors exert their activities in different ways; warfarin inhibits mesangial cell proliferation possibly by inhibiting gamma-carboxylation of Gas6, whereas Axl-Fc blocks the binding of Gas6 to the cell surface Axl by scavenging Gas6.	bind
26675	3	7329	5	13	NULL	NULL	NULL	statement 2	Process		leads to		possibly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_4_1423_s_17	11290560	22  These two inhibitors exert their activities in different ways; warfarin inhibits mesangial cell proliferation possibly by inhibiting gamma-carboxylation of Gas6, whereas Axl-Fc blocks the binding of Gas6 to the cell surface Axl by scavenging Gas6.	bind
26676	4	7329	5	13	NULL	NULL	NULL	Gas6	GP		bind					Axl	GP	cell surface			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_4_1423_s_17	11290560	22  These two inhibitors exert their activities in different ways; warfarin inhibits mesangial cell proliferation possibly by inhibiting gamma-carboxylation of Gas6, whereas Axl-Fc blocks the binding of Gas6 to the cell surface Axl by scavenging Gas6.	bind
26677	5	7329	5	13	NULL	NULL	NULL	Axl-Fc	GP		blocks					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_4_1423_s_17	11290560	22  These two inhibitors exert their activities in different ways; warfarin inhibits mesangial cell proliferation possibly by inhibiting gamma-carboxylation of Gas6, whereas Axl-Fc blocks the binding of Gas6 to the cell surface Axl by scavenging Gas6.	bind
26678	6	7329	5	13	NULL	NULL	NULL	Axl-Fc	GP		scavenges					Gas6	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_4_1423_s_17	11290560	22  These two inhibitors exert their activities in different ways; warfarin inhibits mesangial cell proliferation possibly by inhibiting gamma-carboxylation of Gas6, whereas Axl-Fc blocks the binding of Gas6 to the cell surface Axl by scavenging Gas6.	bind
26679	7	7329	5	13	NULL	NULL	NULL	statement 6	Process		leads to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_4_1423_s_17	11290560	22  These two inhibitors exert their activities in different ways; warfarin inhibits mesangial cell proliferation possibly by inhibiting gamma-carboxylation of Gas6, whereas Axl-Fc blocks the binding of Gas6 to the cell surface Axl by scavenging Gas6.	bind
29117	1	7329	7	10	NULL	0	NULL	 warfarin			inhibits					mesangial cell 		proliferation of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_4_1423_s_17	11290560	22  These two inhibitors exert their activities in different ways; warfarin inhibits mesangial cell proliferation possibly by inhibiting gamma-carboxylation of Gas6, whereas Axl-Fc blocks the binding of Gas6 to the cell surface Axl by scavenging Gas6.	bind
29118	2	7329	7	10	NULL	0	NULL	statement 1			occur by		may			Gas6		 inhibition of;;carboxylation of	gamma		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_4_1423_s_17	11290560	22  These two inhibitors exert their activities in different ways; warfarin inhibits mesangial cell proliferation possibly by inhibiting gamma-carboxylation of Gas6, whereas Axl-Fc blocks the binding of Gas6 to the cell surface Axl by scavenging Gas6.	bind
29119	3	7329	7	NULL	NULL	0	NULL	Gas6	NULL		bind	NULL				 Axl	NULL	cell surface			NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_4_1423_s_17	11290560	22  These two inhibitors exert their activities in different ways; warfarin inhibits mesangial cell proliferation possibly by inhibiting gamma-carboxylation of Gas6, whereas Axl-Fc blocks the binding of Gas6 to the cell surface Axl by scavenging Gas6.	bind
29120	4	7329	7	NULL	NULL	0	NULL	Axl-Fc	NULL		blocks	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_4_1423_s_17	11290560	22  These two inhibitors exert their activities in different ways; warfarin inhibits mesangial cell proliferation possibly by inhibiting gamma-carboxylation of Gas6, whereas Axl-Fc blocks the binding of Gas6 to the cell surface Axl by scavenging Gas6.	bind
29121	5	7329	7	NULL	NULL	0	NULL	statement 3	NULL		occurs by	NULL				Gas6	NULL	scavenging			NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_4_1423_s_17	11290560	22  These two inhibitors exert their activities in different ways; warfarin inhibits mesangial cell proliferation possibly by inhibiting gamma-carboxylation of Gas6, whereas Axl-Fc blocks the binding of Gas6 to the cell surface Axl by scavenging Gas6.	bind
26680	1	7330	5	13	NULL	NULL	NULL	anti-LIBS1	GP	binding of	indicates					fibrinogen receptor	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_94_3_279_s_88	8759067	22  Thus, anti-LIBS1 binding indicates fibrinogen receptor activity.	bind
29122	1	7330	7	NULL	NULL	0	NULL	anti-LIBS1	NULL	binding of	indicates	NULL				fibrinogen receptor	NULL	activity of			NULL		0	NULL	NULL	NULL	gw60_circulation_94_3_279_s_88	8759067	22  Thus, anti-LIBS1 binding indicates fibrinogen receptor activity.	bind
26786	1	7332	5	13	NULL	NULL	NULL	tissue factor	GP		bind					factor VII	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_11_3323_s_24	7586321	22  When exposed to blood, tissue factor binds factors VII and VIIa, resulting in assembly of the functional tissue factor - factor VIIa complex, which in turn activates factors IX and X. 23 24  Factor Xa and its cofactor Va assembled on cell surfaces then convert prothrombin to thrombin.	bind
26787	2	7332	5	13	NULL	NULL	NULL	blood	OrganismPart	exposure to	leads to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_11_3323_s_24	7586321	22  When exposed to blood, tissue factor binds factors VII and VIIa, resulting in assembly of the functional tissue factor - factor VIIa complex, which in turn activates factors IX and X. 23 24  Factor Xa and its cofactor Va assembled on cell surfaces then convert prothrombin to thrombin.	bind
26788	3	7332	5	13	NULL	NULL	NULL	tissue factor	GP		bind					factor VIIa	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_11_3323_s_24	7586321	22  When exposed to blood, tissue factor binds factors VII and VIIa, resulting in assembly of the functional tissue factor - factor VIIa complex, which in turn activates factors IX and X. 23 24  Factor Xa and its cofactor Va assembled on cell surfaces then convert prothrombin to thrombin.	bind
26789	4	7332	5	13	NULL	NULL	NULL	blood	OrganismPart	exposure to	leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_11_3323_s_24	7586321	22  When exposed to blood, tissue factor binds factors VII and VIIa, resulting in assembly of the functional tissue factor - factor VIIa complex, which in turn activates factors IX and X. 23 24  Factor Xa and its cofactor Va assembled on cell surfaces then convert prothrombin to thrombin.	bind
26790	5	7332	5	13	NULL	NULL	NULL	statement 1	Process		assembles					tissue factor - factor VIIa complex	GP	functional			NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_11_3323_s_24	7586321	22  When exposed to blood, tissue factor binds factors VII and VIIa, resulting in assembly of the functional tissue factor - factor VIIa complex, which in turn activates factors IX and X. 23 24  Factor Xa and its cofactor Va assembled on cell surfaces then convert prothrombin to thrombin.	bind
26791	6	7332	5	13	NULL	NULL	NULL	statement 3	Process		assembles					tissue factor - factor VIIa complex	GP	functional			NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_11_3323_s_24	7586321	22  When exposed to blood, tissue factor binds factors VII and VIIa, resulting in assembly of the functional tissue factor - factor VIIa complex, which in turn activates factors IX and X. 23 24  Factor Xa and its cofactor Va assembled on cell surfaces then convert prothrombin to thrombin.	bind
26792	7	7332	5	13	NULL	NULL	NULL	statement 5	Process		activates					factor IX	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_11_3323_s_24	7586321	22  When exposed to blood, tissue factor binds factors VII and VIIa, resulting in assembly of the functional tissue factor - factor VIIa complex, which in turn activates factors IX and X. 23 24  Factor Xa and its cofactor Va assembled on cell surfaces then convert prothrombin to thrombin.	bind
26793	8	7332	5	13	NULL	NULL	NULL	statement 5	Process		activates					factor X	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_11_3323_s_24	7586321	22  When exposed to blood, tissue factor binds factors VII and VIIa, resulting in assembly of the functional tissue factor - factor VIIa complex, which in turn activates factors IX and X. 23 24  Factor Xa and its cofactor Va assembled on cell surfaces then convert prothrombin to thrombin.	bind
26794	9	7332	5	13	NULL	NULL	NULL	statement 6	Process		activates					factor IX	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_11_3323_s_24	7586321	22  When exposed to blood, tissue factor binds factors VII and VIIa, resulting in assembly of the functional tissue factor - factor VIIa complex, which in turn activates factors IX and X. 23 24  Factor Xa and its cofactor Va assembled on cell surfaces then convert prothrombin to thrombin.	bind
26795	10	7332	5	13	NULL	NULL	NULL	statement 6	Process		activates					factor X	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_11_3323_s_24	7586321	22  When exposed to blood, tissue factor binds factors VII and VIIa, resulting in assembly of the functional tissue factor - factor VIIa complex, which in turn activates factors IX and X. 23 24  Factor Xa and its cofactor Va assembled on cell surfaces then convert prothrombin to thrombin.	bind
26796	11	7332	5	13	NULL	NULL	NULL	prothrombin	GP		is converted to					thrombin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_11_3323_s_24	7586321	22  When exposed to blood, tissue factor binds factors VII and VIIa, resulting in assembly of the functional tissue factor - factor VIIa complex, which in turn activates factors IX and X. 23 24  Factor Xa and its cofactor Va assembled on cell surfaces then convert prothrombin to thrombin.	bind
26797	12	7332	5	10	NULL	0	NULL	factor Xa	NULL		is required for	NULL				statement 11	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_11_3323_s_24	7586321	22  When exposed to blood, tissue factor binds factors VII and VIIa, resulting in assembly of the functional tissue factor - factor VIIa complex, which in turn activates factors IX and X. 23 24  Factor Xa and its cofactor Va assembled on cell surfaces then convert prothrombin to thrombin.	bind
26798	13	7332	5	10	NULL	0	NULL	cofactor Va	NULL		is required for	NULL				statement 11	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_11_3323_s_24	7586321	22  When exposed to blood, tissue factor binds factors VII and VIIa, resulting in assembly of the functional tissue factor - factor VIIa complex, which in turn activates factors IX and X. 23 24  Factor Xa and its cofactor Va assembled on cell surfaces then convert prothrombin to thrombin.	bind
46572	14	7332	5	13	NULL	NULL	NULL	Factor Xa	Process		is assembled on					cell surfaces	Cell				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_11_3323_s_24	7586321	22  When exposed to blood, tissue factor binds factors VII and VIIa, resulting in assembly of the functional tissue factor - factor VIIa complex, which in turn activates factors IX and X. 23 24  Factor Xa and its cofactor Va assembled on cell surfaces then convert prothrombin to thrombin.	bind
46573	15	7332	5	10	NULL	0	NULL	cofactor Va	NULL		is assembled on	NULL				cell surface	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_11_3323_s_24	7586321	22  When exposed to blood, tissue factor binds factors VII and VIIa, resulting in assembly of the functional tissue factor - factor VIIa complex, which in turn activates factors IX and X. 23 24  Factor Xa and its cofactor Va assembled on cell surfaces then convert prothrombin to thrombin.	bind
29151	1	7332	7	NULL	NULL	0	NULL	 tissue factor	NULL		binds	NULL				factors VII	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_11_3323_s_24	7586321	22  When exposed to blood, tissue factor binds factors VII and VIIa, resulting in assembly of the functional tissue factor - factor VIIa complex, which in turn activates factors IX and X. 23 24  Factor Xa and its cofactor Va assembled on cell surfaces then convert prothrombin to thrombin.	bind
29153	2	7332	7	NULL	NULL	0	NULL	tissue factor	NULL		binds	NULL				factor VIIa	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_11_3323_s_24	7586321	22  When exposed to blood, tissue factor binds factors VII and VIIa, resulting in assembly of the functional tissue factor - factor VIIa complex, which in turn activates factors IX and X. 23 24  Factor Xa and its cofactor Va assembled on cell surfaces then convert prothrombin to thrombin.	bind
29155	3	7332	7	NULL	NULL	0	NULL	statement 1	NULL		occurs when	NULL				blood 	NULL	exposed to			NULL		0	NULL	NULL	NULL	gw60_circulation_92_11_3323_s_24	7586321	22  When exposed to blood, tissue factor binds factors VII and VIIa, resulting in assembly of the functional tissue factor - factor VIIa complex, which in turn activates factors IX and X. 23 24  Factor Xa and its cofactor Va assembled on cell surfaces then convert prothrombin to thrombin.	bind
29156	4	7332	7	NULL	NULL	0	NULL	statement 2	NULL		occurs when	NULL				blood	NULL	exposed to			NULL		0	NULL	NULL	NULL	gw60_circulation_92_11_3323_s_24	7586321	22  When exposed to blood, tissue factor binds factors VII and VIIa, resulting in assembly of the functional tissue factor - factor VIIa complex, which in turn activates factors IX and X. 23 24  Factor Xa and its cofactor Va assembled on cell surfaces then convert prothrombin to thrombin.	bind
29158	5	7332	7	NULL	NULL	0	NULL	statement 1	NULL		assembles 	NULL				tissue factor - factor VIIa complex	NULL	 functional			NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_11_3323_s_24	7586321	22  When exposed to blood, tissue factor binds factors VII and VIIa, resulting in assembly of the functional tissue factor - factor VIIa complex, which in turn activates factors IX and X. 23 24  Factor Xa and its cofactor Va assembled on cell surfaces then convert prothrombin to thrombin.	bind
29161	6	7332	7	NULL	NULL	0	NULL	statement 2	NULL		assembles 	NULL				tissue factor - factor VIIa complex	NULL	functional			NULL		0	NULL	NULL	NULL	gw60_circulation_92_11_3323_s_24	7586321	22  When exposed to blood, tissue factor binds factors VII and VIIa, resulting in assembly of the functional tissue factor - factor VIIa complex, which in turn activates factors IX and X. 23 24  Factor Xa and its cofactor Va assembled on cell surfaces then convert prothrombin to thrombin.	bind
29162	7	7332	7	NULL	NULL	0	NULL	statement 5	NULL		activates	NULL				 factors IX	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_11_3323_s_24	7586321	22  When exposed to blood, tissue factor binds factors VII and VIIa, resulting in assembly of the functional tissue factor - factor VIIa complex, which in turn activates factors IX and X. 23 24  Factor Xa and its cofactor Va assembled on cell surfaces then convert prothrombin to thrombin.	bind
29163	8	7332	7	NULL	NULL	0	NULL	statement 6	NULL		activates	NULL				factor IX	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_11_3323_s_24	7586321	22  When exposed to blood, tissue factor binds factors VII and VIIa, resulting in assembly of the functional tissue factor - factor VIIa complex, which in turn activates factors IX and X. 23 24  Factor Xa and its cofactor Va assembled on cell surfaces then convert prothrombin to thrombin.	bind
29164	9	7332	7	NULL	NULL	0	NULL	statement 5	NULL		activates	NULL				factor X	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_11_3323_s_24	7586321	22  When exposed to blood, tissue factor binds factors VII and VIIa, resulting in assembly of the functional tissue factor - factor VIIa complex, which in turn activates factors IX and X. 23 24  Factor Xa and its cofactor Va assembled on cell surfaces then convert prothrombin to thrombin.	bind
29165	10	7332	7	NULL	NULL	0	NULL	statement 6	NULL		activates	NULL				factor X	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_11_3323_s_24	7586321	22  When exposed to blood, tissue factor binds factors VII and VIIa, resulting in assembly of the functional tissue factor - factor VIIa complex, which in turn activates factors IX and X. 23 24  Factor Xa and its cofactor Va assembled on cell surfaces then convert prothrombin to thrombin.	bind
29166	11	7332	7	NULL	NULL	0	NULL	Factor Xa	NULL		assemble on	NULL				cell surface	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_11_3323_s_24	7586321	22  When exposed to blood, tissue factor binds factors VII and VIIa, resulting in assembly of the functional tissue factor - factor VIIa complex, which in turn activates factors IX and X. 23 24  Factor Xa and its cofactor Va assembled on cell surfaces then convert prothrombin to thrombin.	bind
29169	12	7332	7	NULL	NULL	0	NULL	cofactor Va	NULL		assemble on	NULL				cell surface	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_11_3323_s_24	7586321	22  When exposed to blood, tissue factor binds factors VII and VIIa, resulting in assembly of the functional tissue factor - factor VIIa complex, which in turn activates factors IX and X. 23 24  Factor Xa and its cofactor Va assembled on cell surfaces then convert prothrombin to thrombin.	bind
29173	13	7332	7	NULL	NULL	0	NULL	prothrombin	NULL		converts to	NULL				thrombin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_11_3323_s_24	7586321	22  When exposed to blood, tissue factor binds factors VII and VIIa, resulting in assembly of the functional tissue factor - factor VIIa complex, which in turn activates factors IX and X. 23 24  Factor Xa and its cofactor Va assembled on cell surfaces then convert prothrombin to thrombin.	bind
29175	14	7332	7	NULL	NULL	0	NULL	statement 11	NULL		converts 	NULL				statement 13	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_11_3323_s_24	7586321	22  When exposed to blood, tissue factor binds factors VII and VIIa, resulting in assembly of the functional tissue factor - factor VIIa complex, which in turn activates factors IX and X. 23 24  Factor Xa and its cofactor Va assembled on cell surfaces then convert prothrombin to thrombin.	bind
29178	15	7332	7	NULL	NULL	0	NULL	statement 12	NULL		converts	NULL				statement 13	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_11_3323_s_24	7586321	22  When exposed to blood, tissue factor binds factors VII and VIIa, resulting in assembly of the functional tissue factor - factor VIIa complex, which in turn activates factors IX and X. 23 24  Factor Xa and its cofactor Va assembled on cell surfaces then convert prothrombin to thrombin.	bind
26799	1	7333	5	13	NULL	NULL	NULL	HSBP1	GP		is					hsp binding factor 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_8_1012_s_27	11864934	22 A second mechanism involves an interaction between hsp binding factor 1 (HSBP1) with the active trimeric form of HSF1 and hsp70, thereby inhibiting the capacity of HSF1 to bind to DNA. 23	bind
26800	2	7333	5	13	NULL	NULL	NULL	HSBP1	GP		interacts with					HSF1	GP	active trimeric form of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_8_1012_s_27	11864934	22 A second mechanism involves an interaction between hsp binding factor 1 (HSBP1) with the active trimeric form of HSF1 and hsp70, thereby inhibiting the capacity of HSF1 to bind to DNA. 23	bind
26801	3	7333	5	13	NULL	NULL	NULL	HSBP1	GP		interacts with					hsp70	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_8_1012_s_27	11864934	22 A second mechanism involves an interaction between hsp binding factor 1 (HSBP1) with the active trimeric form of HSF1 and hsp70, thereby inhibiting the capacity of HSF1 to bind to DNA. 23	bind
26802	4	7333	5	13	NULL	NULL	NULL	HSF1	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_8_1012_s_27	11864934	22 A second mechanism involves an interaction between hsp binding factor 1 (HSBP1) with the active trimeric form of HSF1 and hsp70, thereby inhibiting the capacity of HSF1 to bind to DNA. 23	bind
26803	5	7333	5	13	NULL	NULL	NULL	statement 2	Process		inhibit					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_8_1012_s_27	11864934	22 A second mechanism involves an interaction between hsp binding factor 1 (HSBP1) with the active trimeric form of HSF1 and hsp70, thereby inhibiting the capacity of HSF1 to bind to DNA. 23	bind
26804	6	7333	5	13	NULL	NULL	NULL	statement 3	Process		inhibit					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_8_1012_s_27	11864934	22 A second mechanism involves an interaction between hsp binding factor 1 (HSBP1) with the active trimeric form of HSF1 and hsp70, thereby inhibiting the capacity of HSF1 to bind to DNA. 23	bind
29182	1	7333	7	NULL	NULL	0	NULL	HSBP1	NULL		interacts with	NULL				HSF1	NULL	active trimeric form of			NULL		0	NULL	NULL	NULL	gw60_circulation_105_8_1012_s_27	11864934	22 A second mechanism involves an interaction between hsp binding factor 1 (HSBP1) with the active trimeric form of HSF1 and hsp70, thereby inhibiting the capacity of HSF1 to bind to DNA. 23	bind
29183	2	7333	7	NULL	NULL	0	NULL	HSBP1	NULL		interacts with	NULL				hsp70	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_8_1012_s_27	11864934	22 A second mechanism involves an interaction between hsp binding factor 1 (HSBP1) with the active trimeric form of HSF1 and hsp70, thereby inhibiting the capacity of HSF1 to bind to DNA. 23	bind
29184	3	7333	7	NULL	NULL	0	NULL	HSF1	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_8_1012_s_27	11864934	22 A second mechanism involves an interaction between hsp binding factor 1 (HSBP1) with the active trimeric form of HSF1 and hsp70, thereby inhibiting the capacity of HSF1 to bind to DNA. 23	bind
29185	4	7333	7	NULL	NULL	0	NULL	statement 1	NULL		inhibit	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_8_1012_s_27	11864934	22 A second mechanism involves an interaction between hsp binding factor 1 (HSBP1) with the active trimeric form of HSF1 and hsp70, thereby inhibiting the capacity of HSF1 to bind to DNA. 23	bind
29186	5	7333	7	NULL	NULL	0	NULL	statement 2	NULL		inhibit	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_8_1012_s_27	11864934	22 A second mechanism involves an interaction between hsp binding factor 1 (HSBP1) with the active trimeric form of HSF1 and hsp70, thereby inhibiting the capacity of HSF1 to bind to DNA. 23	bind
29223	6	7333	7	NULL	NULL	0	NULL	HSBP1	NULL		is	NULL				hsp binding factor 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_8_1012_s_27	11864934	22 A second mechanism involves an interaction between hsp binding factor 1 (HSBP1) with the active trimeric form of HSF1 and hsp70, thereby inhibiting the capacity of HSF1 to bind to DNA. 23	bind
26805	1	7334	5	13	NULL	NULL	NULL	Rac1	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_3_276_s_29	15217908	22 Although originally posited to be a GAP based on its amino acid sequence similarity to Ras-GAP, subsequent in vitro analysis revealed that IQGAP1 binds to active (GTP-bound) Rac1, which in turn inhibits its intrinsic GTPase activity, thereby increasing active Rac1.	bind
26806	2	7334	5	13	NULL	NULL	NULL	IQGAP1	GP		bind					statement 1	Process	active			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_circulationres_95_3_276_s_29	15217908	22 Although originally posited to be a GAP based on its amino acid sequence similarity to Ras-GAP, subsequent in vitro analysis revealed that IQGAP1 binds to active (GTP-bound) Rac1, which in turn inhibits its intrinsic GTPase activity, thereby increasing active Rac1.	bind
26807	3	7334	5	13	NULL	NULL	NULL	statement 2	Process		inhibit					GTPase 	GP	intrinsic activity of			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_circulationres_95_3_276_s_29	15217908	22 Although originally posited to be a GAP based on its amino acid sequence similarity to Ras-GAP, subsequent in vitro analysis revealed that IQGAP1 binds to active (GTP-bound) Rac1, which in turn inhibits its intrinsic GTPase activity, thereby increasing active Rac1.	bind
26808	4	7334	5	13	NULL	NULL	NULL	statement 3	Process		increases					Rac1	GP	active			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_circulationres_95_3_276_s_29	15217908	22 Although originally posited to be a GAP based on its amino acid sequence similarity to Ras-GAP, subsequent in vitro analysis revealed that IQGAP1 binds to active (GTP-bound) Rac1, which in turn inhibits its intrinsic GTPase activity, thereby increasing active Rac1.	bind
29187	1	7334	7	10	NULL	0	NULL	GTP			binds to					Rac1					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_3_276_s_29	15217908	22 Although originally posited to be a GAP based on its amino acid sequence similarity to Ras-GAP, subsequent in vitro analysis revealed that IQGAP1 binds to active (GTP-bound) Rac1, which in turn inhibits its intrinsic GTPase activity, thereby increasing active Rac1.	bind
29188	2	7334	7	NULL	NULL	0	NULL	statement 1	NULL		inhibits	NULL				GTPase	NULL	intrinsic activity of			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_circulationres_95_3_276_s_29	15217908	22 Although originally posited to be a GAP based on its amino acid sequence similarity to Ras-GAP, subsequent in vitro analysis revealed that IQGAP1 binds to active (GTP-bound) Rac1, which in turn inhibits its intrinsic GTPase activity, thereby increasing active Rac1.	bind
29189	3	7334	7	NULL	NULL	0	NULL	statement 2	NULL		increase	NULL				Rac1	NULL	active			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_circulationres_95_3_276_s_29	15217908	22 Although originally posited to be a GAP based on its amino acid sequence similarity to Ras-GAP, subsequent in vitro analysis revealed that IQGAP1 binds to active (GTP-bound) Rac1, which in turn inhibits its intrinsic GTPase activity, thereby increasing active Rac1.	bind
46574	4	7334	7	10	NULL	0	NULL	IQGAP1			bind					statement 1					NULL	in vitro	NULL	NULL	NULL	NULL	gw70_circulationres_95_3_276_s_29	15217908	22 Although originally posited to be a GAP based on its amino acid sequence similarity to Ras-GAP, subsequent in vitro analysis revealed that IQGAP1 binds to active (GTP-bound) Rac1, which in turn inhibits its intrinsic GTPase activity, thereby increasing active Rac1.	bind
26809	1	7335	5	13	NULL	NULL	NULL	LDLR	GP		bind					apoE	GP	newly synthesized			NULL	in macrophages	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_91_s_161	12969990	22 Although the role of LDLR in these processes has not been addressed, LDLR is known to bind to newly synthesized apoE in macrophages and limits its secretion.	bind
26810	2	7335	5	13	NULL	NULL	NULL	statement 1	Process		limits					apoE	GP	secretion of			NULL	macrophages	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_91_s_161	12969990	22 Although the role of LDLR in these processes has not been addressed, LDLR is known to bind to newly synthesized apoE in macrophages and limits its secretion.	bind
29190	1	7335	7	NULL	NULL	0	NULL	 LDLR 	NULL		binds	NULL				apoE	NULL	newly synthesized			NULL	macrophages	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_91_s_161	12969990	22 Although the role of LDLR in these processes has not been addressed, LDLR is known to bind to newly synthesized apoE in macrophages and limits its secretion.	bind
29191	2	7335	7	10	NULL	0	NULL	statement 1			limits					apoE		secretion of			NULL	macrophages	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_91_s_161	12969990	22 Although the role of LDLR in these processes has not been addressed, LDLR is known to bind to newly synthesized apoE in macrophages and limits its secretion.	bind
26811	1	7336	5	13	NULL	NULL	NULL				plays a role in				CArG elements	SRF	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1596_s_154	15231515	22 It is also possible that subtle difference in DNA sequences within the CArG elements may play a role in determining not only SRF binding, 26 but also subsequent recruitment of myocardin.	bind
26812	2	7336	5	13	NULL	NULL	NULL				plays a role in				CArG elements	myocardin	GP	recruitment of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1596_s_154	15231515	22 It is also possible that subtle difference in DNA sequences within the CArG elements may play a role in determining not only SRF binding, 26 but also subsequent recruitment of myocardin.	bind
29192	1	7336	7	NULL	NULL	0	NULL		NULL		plays a role in	NULL			 CArG elements	SRF	NULL	binding of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1596_s_154	15231515	22 It is also possible that subtle difference in DNA sequences within the CArG elements may play a role in determining not only SRF binding, 26 but also subsequent recruitment of myocardin.	bind
29193	2	7336	7	NULL	NULL	0	NULL		NULL		plays a role in	NULL			CArG elements	myocardin	NULL	recruitment of 			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1596_s_154	15231515	22 It is also possible that subtle difference in DNA sequences within the CArG elements may play a role in determining not only SRF binding, 26 but also subsequent recruitment of myocardin.	bind
26813	1	7337	5	13	NULL	NULL	NULL	PTX3	GP		bind					FGF2	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_9_1837_s_33	16020751	22 Moreover, PTX3 binds FGF2 and inhibits its angiogenic activity on endothelial cells.	bind
26814	2	7337	5	13	NULL	NULL	NULL	FGF2	GP		exhibits					angiogenic activity	Process				NULL	on endothelial cells	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_9_1837_s_33	16020751	22 Moreover, PTX3 binds FGF2 and inhibits its angiogenic activity on endothelial cells.	bind
46575	3	7337	5	13	NULL	NULL	NULL	statement 1	Process		inhibits					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_9_1837_s_33	16020751	22 Moreover, PTX3 binds FGF2 and inhibits its angiogenic activity on endothelial cells.	bind
29194	1	7337	7	NULL	NULL	0	NULL	PTX3	NULL		binds	NULL				FGF2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_9_1837_s_33	16020751	22 Moreover, PTX3 binds FGF2 and inhibits its angiogenic activity on endothelial cells.	bind
29195	2	7337	7	10	NULL	0	NULL	FGF2	NULL		exhibits	NULL				angiogenic activity	NULL				NULL	endothelial cells	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_9_1837_s_33	16020751	22 Moreover, PTX3 binds FGF2 and inhibits its angiogenic activity on endothelial cells.	bind
46576	3	7337	7	10	NULL	0	NULL	statement 1	NULL		inhibits	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_9_1837_s_33	16020751	22 Moreover, PTX3 binds FGF2 and inhibits its angiogenic activity on endothelial cells.	bind
26815	1	7338	5	13	NULL	NULL	NULL	PKC	GP	activation of	cause		might			insulin resistance	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_28_s_42	16239592	22 The activation of PKC might cause insulin resistance by ultimately inducing serine/tyrosine phosphorylation of insulin receptor substrate 1 (IRS-1) sites, thereby inhibiting IRS-1 binding and activation of phosphoinositol 3-kinase.	bind
26816	2	7338	5	13	NULL	NULL	NULL	IRS-1	GP		is					insulin receptor substrate 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_28_s_42	16239592	22 The activation of PKC might cause insulin resistance by ultimately inducing serine/tyrosine phosphorylation of insulin receptor substrate 1 (IRS-1) sites, thereby inhibiting IRS-1 binding and activation of phosphoinositol 3-kinase.	bind
26817	3	7338	5	13	NULL	NULL	NULL	statement 1	Process		induces					IRS-1	GP	phosphorylation of	serine/tyrosine		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_28_s_42	16239592	22 The activation of PKC might cause insulin resistance by ultimately inducing serine/tyrosine phosphorylation of insulin receptor substrate 1 (IRS-1) sites, thereby inhibiting IRS-1 binding and activation of phosphoinositol 3-kinase.	bind
26818	4	7338	5	13	NULL	NULL	NULL	statement 3	Process		inhibit					IRS-1	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_28_s_42	16239592	22 The activation of PKC might cause insulin resistance by ultimately inducing serine/tyrosine phosphorylation of insulin receptor substrate 1 (IRS-1) sites, thereby inhibiting IRS-1 binding and activation of phosphoinositol 3-kinase.	bind
26819	5	7338	5	13	NULL	NULL	NULL	statement 3	Process		inhibit					phosphoinositol 3-kinase	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_28_s_42	16239592	22 The activation of PKC might cause insulin resistance by ultimately inducing serine/tyrosine phosphorylation of insulin receptor substrate 1 (IRS-1) sites, thereby inhibiting IRS-1 binding and activation of phosphoinositol 3-kinase.	bind
29196	1	7338	7	NULL	NULL	0	NULL	PKC	NULL	activation of	cause	NULL				insulin resistance	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_28_s_42	16239592	22 The activation of PKC might cause insulin resistance by ultimately inducing serine/tyrosine phosphorylation of insulin receptor substrate 1 (IRS-1) sites, thereby inhibiting IRS-1 binding and activation of phosphoinositol 3-kinase.	bind
29197	2	7338	7	NULL	NULL	0	NULL	statement 1	NULL		induce	NULL				IRS-1	NULL	phosphorylation of	serine/tyrosine sites		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_28_s_42	16239592	22 The activation of PKC might cause insulin resistance by ultimately inducing serine/tyrosine phosphorylation of insulin receptor substrate 1 (IRS-1) sites, thereby inhibiting IRS-1 binding and activation of phosphoinositol 3-kinase.	bind
29198	3	7338	7	10	NULL	0	NULL	IRS-1			is					insulin receptor substrate 1					NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_28_s_42	16239592	22 The activation of PKC might cause insulin resistance by ultimately inducing serine/tyrosine phosphorylation of insulin receptor substrate 1 (IRS-1) sites, thereby inhibiting IRS-1 binding and activation of phosphoinositol 3-kinase.	bind
29199	4	7338	7	NULL	NULL	0	NULL	statement 2	NULL		activates	NULL				phosphoinositol 3-kinase	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_28_s_42	16239592	22 The activation of PKC might cause insulin resistance by ultimately inducing serine/tyrosine phosphorylation of insulin receptor substrate 1 (IRS-1) sites, thereby inhibiting IRS-1 binding and activation of phosphoinositol 3-kinase.	bind
29200	5	7338	7	NULL	NULL	0	NULL	statement 2	NULL		inhibits	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_28_s_42	16239592	22 The activation of PKC might cause insulin resistance by ultimately inducing serine/tyrosine phosphorylation of insulin receptor substrate 1 (IRS-1) sites, thereby inhibiting IRS-1 binding and activation of phosphoinositol 3-kinase.	bind
26820	1	7339	5	13	NULL	NULL	NULL	heparin	Chemical		decrease		may			RLP-SMC	Process	interaction of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_108_21_2679_s_152	14623816	22 Thus, heparin and heparitinase may not only decrease RLP-SMC interaction but also interfere with the binding of soluble HB-EGF generated by RLPs to EGF receptor.	bind
26821	2	7339	5	13	NULL	NULL	NULL	heparitinase	GP		decreases		may			RLP-SMC	Process	interaction of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_108_21_2679_s_152	14623816	22 Thus, heparin and heparitinase may not only decrease RLP-SMC interaction but also interfere with the binding of soluble HB-EGF generated by RLPs to EGF receptor.	bind
26822	3	7339	5	13	NULL	NULL	NULL	HB-EGF	GP	soluble	is generated by					RLPs	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_108_21_2679_s_152	14623816	22 Thus, heparin and heparitinase may not only decrease RLP-SMC interaction but also interfere with the binding of soluble HB-EGF generated by RLPs to EGF receptor.	bind
26823	4	7339	5	13	NULL	NULL	NULL	statement 3	GP		bind					EGF receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_108_21_2679_s_152	14623816	22 Thus, heparin and heparitinase may not only decrease RLP-SMC interaction but also interfere with the binding of soluble HB-EGF generated by RLPs to EGF receptor.	bind
26824	5	7339	5	13	NULL	NULL	NULL	heparin	Chemical		interferes with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_108_21_2679_s_152	14623816	22 Thus, heparin and heparitinase may not only decrease RLP-SMC interaction but also interfere with the binding of soluble HB-EGF generated by RLPs to EGF receptor.	bind
26825	6	7339	5	13	NULL	NULL	NULL	heparitinase	GP		interferes with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_108_21_2679_s_152	14623816	22 Thus, heparin and heparitinase may not only decrease RLP-SMC interaction but also interfere with the binding of soluble HB-EGF generated by RLPs to EGF receptor.	bind
29201	1	7339	7	NULL	NULL	0	NULL	RLP	NULL		interacts with	NULL				SMC	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_108_21_2679_s_152	14623816	22 Thus, heparin and heparitinase may not only decrease RLP-SMC interaction but also interfere with the binding of soluble HB-EGF generated by RLPs to EGF receptor.	bind
29202	2	7339	7	NULL	NULL	0	NULL	HB-EGF	NULL	soluble	binds to	NULL				EGF receptor	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_108_21_2679_s_152	14623816	22 Thus, heparin and heparitinase may not only decrease RLP-SMC interaction but also interfere with the binding of soluble HB-EGF generated by RLPs to EGF receptor.	bind
29203	3	7339	7	NULL	NULL	0	NULL	heparin	NULL		decrease	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulation_108_21_2679_s_152	14623816	22 Thus, heparin and heparitinase may not only decrease RLP-SMC interaction but also interfere with the binding of soluble HB-EGF generated by RLPs to EGF receptor.	bind
29204	4	7339	7	NULL	NULL	0	NULL	heparitinase	NULL		decrease	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulation_108_21_2679_s_152	14623816	22 Thus, heparin and heparitinase may not only decrease RLP-SMC interaction but also interfere with the binding of soluble HB-EGF generated by RLPs to EGF receptor.	bind
29205	5	7339	7	NULL	NULL	0	NULL	heparin	NULL		interferes with	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulation_108_21_2679_s_152	14623816	22 Thus, heparin and heparitinase may not only decrease RLP-SMC interaction but also interfere with the binding of soluble HB-EGF generated by RLPs to EGF receptor.	bind
29206	6	7339	7	NULL	NULL	0	NULL	heparitinase	NULL		interferes with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_108_21_2679_s_152	14623816	22 Thus, heparin and heparitinase may not only decrease RLP-SMC interaction but also interfere with the binding of soluble HB-EGF generated by RLPs to EGF receptor.	bind
29207	7	7339	7	NULL	NULL	0	NULL	RLP	NULL		generates	NULL				HB-EGF	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_108_21_2679_s_152	14623816	22 Thus, heparin and heparitinase may not only decrease RLP-SMC interaction but also interfere with the binding of soluble HB-EGF generated by RLPs to EGF receptor.	bind
26826	1	7340	5	13	NULL	NULL	NULL	elastin	GP		mediate					calcification	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_6_1981_s_143	11733347	22 With respect to elastin-mediated calcification, both MMP-2 and MMP-9 are known to bind insoluble elastin, 8  and each have been shown to be actively involved in elastin degradation.	bind
26827	2	7340	5	13	NULL	NULL	NULL	MMP-2	GP		bind					elastin	GP	insoluble			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_6_1981_s_143	11733347	22 With respect to elastin-mediated calcification, both MMP-2 and MMP-9 are known to bind insoluble elastin, 8  and each have been shown to be actively involved in elastin degradation.	bind
26828	3	7340	5	13	NULL	NULL	NULL	MMP-9	GP		bind					elastin	GP	insoluble			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_6_1981_s_143	11733347	22 With respect to elastin-mediated calcification, both MMP-2 and MMP-9 are known to bind insoluble elastin, 8  and each have been shown to be actively involved in elastin degradation.	bind
26829	4	7340	5	13	NULL	NULL	NULL	MMP-2	GP		is involved in		actively			elastin	GP	degradation of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_6_1981_s_143	11733347	22 With respect to elastin-mediated calcification, both MMP-2 and MMP-9 are known to bind insoluble elastin, 8  and each have been shown to be actively involved in elastin degradation.	bind
26830	5	7340	5	13	NULL	NULL	NULL	MMP-9	GP		is involved in		actively			elastin	GP	degradation of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_6_1981_s_143	11733347	22 With respect to elastin-mediated calcification, both MMP-2 and MMP-9 are known to bind insoluble elastin, 8  and each have been shown to be actively involved in elastin degradation.	bind
29208	1	7340	7	NULL	NULL	0	NULL	MMP-2	NULL		bind	NULL				elastin	NULL	insoluble			NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_6_1981_s_143	11733347	22 With respect to elastin-mediated calcification, both MMP-2 and MMP-9 are known to bind insoluble elastin, 8  and each have been shown to be actively involved in elastin degradation.	bind
29209	2	7340	7	NULL	NULL	0	NULL	MMP-9	NULL		bind	NULL				elastin	NULL	insoluble			NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_6_1981_s_143	11733347	22 With respect to elastin-mediated calcification, both MMP-2 and MMP-9 are known to bind insoluble elastin, 8  and each have been shown to be actively involved in elastin degradation.	bind
29210	3	7340	7	NULL	NULL	0	NULL	MMP-2	NULL		involved in	NULL	actively			elastin	NULL	degradation of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_6_1981_s_143	11733347	22 With respect to elastin-mediated calcification, both MMP-2 and MMP-9 are known to bind insoluble elastin, 8  and each have been shown to be actively involved in elastin degradation.	bind
29211	4	7340	7	NULL	NULL	0	NULL	MMP-9	NULL		 involved in	NULL	actively			elastin	NULL	degradation of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_6_1981_s_143	11733347	22 With respect to elastin-mediated calcification, both MMP-2 and MMP-9 are known to bind insoluble elastin, 8  and each have been shown to be actively involved in elastin degradation.	bind
29212	5	7340	7	NULL	NULL	0	NULL	elastin	NULL		mediates	NULL				calcification	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_6_1981_s_143	11733347	22 With respect to elastin-mediated calcification, both MMP-2 and MMP-9 are known to bind insoluble elastin, 8  and each have been shown to be actively involved in elastin degradation.	bind
26831	1	7341	5	13	NULL	NULL	NULL	NO	Chemical	low levels of	is implicated in					lymphocyte	Cell	activation of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_905_s_16	11891189	22, 23 Low levels of NO have also been implicated in lymphocyte activation and proliferation, increasing TNF-alpha production, nuclear factor-kappaB binding activity, and enhancing tyrosine kinase p56 activity.	bind
26832	2	7341	5	13	NULL	NULL	NULL	NO	Chemical	low levels of	is implicated in					lymphocyte	Cell	proliferation of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_905_s_16	11891189	22, 23 Low levels of NO have also been implicated in lymphocyte activation and proliferation, increasing TNF-alpha production, nuclear factor-kappaB binding activity, and enhancing tyrosine kinase p56 activity.	bind
26833	3	7341	5	13	NULL	NULL	NULL	NO	Chemical	low levels of	is implicated in					TNF-alpha	GP	increasing production of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_905_s_16	11891189	22, 23 Low levels of NO have also been implicated in lymphocyte activation and proliferation, increasing TNF-alpha production, nuclear factor-kappaB binding activity, and enhancing tyrosine kinase p56 activity.	bind
26834	4	7341	5	13	NULL	NULL	NULL	NO	Chemical	low levels of	is implicated in					nuclear factor-kappaB	GP	binding activity of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_905_s_16	11891189	22, 23 Low levels of NO have also been implicated in lymphocyte activation and proliferation, increasing TNF-alpha production, nuclear factor-kappaB binding activity, and enhancing tyrosine kinase p56 activity.	bind
26835	5	7341	5	13	NULL	NULL	NULL	NO	Chemical	low levels of	is implicated in					tyrosine kinase p56	GP	enhancing activity of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_905_s_16	11891189	22, 23 Low levels of NO have also been implicated in lymphocyte activation and proliferation, increasing TNF-alpha production, nuclear factor-kappaB binding activity, and enhancing tyrosine kinase p56 activity.	bind
29213	1	7341	7	NULL	NULL	0	NULL	NO	NULL	low levels of	is implicated in	NULL				lymphocyte	NULL	activation of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_905_s_16	11891189	22, 23 Low levels of NO have also been implicated in lymphocyte activation and proliferation, increasing TNF-alpha production, nuclear factor-kappaB binding activity, and enhancing tyrosine kinase p56 activity.	bind
29214	2	7341	7	NULL	NULL	0	NULL	NO	NULL	low levels of	implicated in	NULL				lymphocyte	NULL	proliferation of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_3_905_s_16	11891189	22, 23 Low levels of NO have also been implicated in lymphocyte activation and proliferation, increasing TNF-alpha production, nuclear factor-kappaB binding activity, and enhancing tyrosine kinase p56 activity.	bind
29215	3	7341	7	NULL	NULL	0	NULL	NO	NULL	low levels of	increase	NULL				TNF-alpha	NULL	production of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_3_905_s_16	11891189	22, 23 Low levels of NO have also been implicated in lymphocyte activation and proliferation, increasing TNF-alpha production, nuclear factor-kappaB binding activity, and enhancing tyrosine kinase p56 activity.	bind
29216	4	7341	7	NULL	NULL	0	NULL	NO	NULL	low levels of	increase	NULL				 nuclear factor-kappaB	NULL	binding activity of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_3_905_s_16	11891189	22, 23 Low levels of NO have also been implicated in lymphocyte activation and proliferation, increasing TNF-alpha production, nuclear factor-kappaB binding activity, and enhancing tyrosine kinase p56 activity.	bind
29217	5	7341	7	NULL	NULL	0	NULL	NO	NULL	low levels of	enhance	NULL				tyrosine kinase p56 	NULL	activity of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_3_905_s_16	11891189	22, 23 Low levels of NO have also been implicated in lymphocyte activation and proliferation, increasing TNF-alpha production, nuclear factor-kappaB binding activity, and enhancing tyrosine kinase p56 activity.	bind
26836	1	7343	5	13	NULL	NULL	NULL	IFN-gammaR	GP		is					IFN-gamma receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_5_1549_s_26	10329607	22- 27  However, it is still unresolved whether IFN-gamma, which binds to the IFN-gamma receptor (IFN-gammaR), and/or TNF-alpha, which binds to the TNFR1 in its soluble form 28  and to the TNFR2 in its membranous form, 29  are crucial for the activation of cerebral endothelium, microglia, and astrocytes  in vivo.	bind
26837	2	7343	5	13	NULL	NULL	NULL	IFN-gamma	GP		bind					IFN-gammaR	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_5_1549_s_26	10329607	22- 27  However, it is still unresolved whether IFN-gamma, which binds to the IFN-gamma receptor (IFN-gammaR), and/or TNF-alpha, which binds to the TNFR1 in its soluble form 28  and to the TNFR2 in its membranous form, 29  are crucial for the activation of cerebral endothelium, microglia, and astrocytes  in vivo.	bind
26838	3	7343	5	13	NULL	NULL	NULL	TNF-alpha	GP		bind					TNFR1	GP	soluble			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_5_1549_s_26	10329607	22- 27  However, it is still unresolved whether IFN-gamma, which binds to the IFN-gamma receptor (IFN-gammaR), and/or TNF-alpha, which binds to the TNFR1 in its soluble form 28  and to the TNFR2 in its membranous form, 29  are crucial for the activation of cerebral endothelium, microglia, and astrocytes  in vivo.	bind
26839	4	7343	5	13	NULL	NULL	NULL	TNF-alpha	GP		bind					TNFR2	GP	membranous form			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_5_1549_s_26	10329607	22- 27  However, it is still unresolved whether IFN-gamma, which binds to the IFN-gamma receptor (IFN-gammaR), and/or TNF-alpha, which binds to the TNFR1 in its soluble form 28  and to the TNFR2 in its membranous form, 29  are crucial for the activation of cerebral endothelium, microglia, and astrocytes  in vivo.	bind
29219	1	7343	7	NULL	NULL	0	NULL	IFN-gamma	NULL		binds to	NULL				IFN-gammaR	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_5_1549_s_26	10329607	22- 27  However, it is still unresolved whether IFN-gamma, which binds to the IFN-gamma receptor (IFN-gammaR), and/or TNF-alpha, which binds to the TNFR1 in its soluble form 28  and to the TNFR2 in its membranous form, 29  are crucial for the activation of cerebral endothelium, microglia, and astrocytes  in vivo.	bind
29220	2	7343	7	NULL	NULL	0	NULL	TNF-alpha	NULL		binds to	NULL				TNFR1	NULL	soluble form			NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_5_1549_s_26	10329607	22- 27  However, it is still unresolved whether IFN-gamma, which binds to the IFN-gamma receptor (IFN-gammaR), and/or TNF-alpha, which binds to the TNFR1 in its soluble form 28  and to the TNFR2 in its membranous form, 29  are crucial for the activation of cerebral endothelium, microglia, and astrocytes  in vivo.	bind
29221	3	7343	7	NULL	NULL	0	NULL	TNF-alpha	NULL		binds to	NULL				TNFR2	NULL	membranous form			NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_5_1549_s_26	10329607	22- 27  However, it is still unresolved whether IFN-gamma, which binds to the IFN-gamma receptor (IFN-gammaR), and/or TNF-alpha, which binds to the TNFR1 in its soluble form 28  and to the TNFR2 in its membranous form, 29  are crucial for the activation of cerebral endothelium, microglia, and astrocytes  in vivo.	bind
29222	4	7343	7	NULL	NULL	0	NULL	IFN-gammaR	NULL		is	NULL				IFN-gamma receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_5_1549_s_26	10329607	22- 27  However, it is still unresolved whether IFN-gamma, which binds to the IFN-gamma receptor (IFN-gammaR), and/or TNF-alpha, which binds to the TNFR1 in its soluble form 28  and to the TNFR2 in its membranous form, 29  are crucial for the activation of cerebral endothelium, microglia, and astrocytes  in vivo.	bind
26840	1	7344	5	13	NULL	NULL	NULL	HLA-E leader sequence	GP		does not bind			MVDGTLLLL		HLA-E	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_currbiol_8_1_1_s_90	9427624	221 cells at 26 degrees C in the presence of exogenous added peptides: MVDGTLLLL from HLA-E leader sequence which is not capable of binding to HLA-E  in vitro and VMAPRTVLL from HLA-B 0801 which can bind to HLA-E.	bind
26841	2	7344	5	13	NULL	NULL	NULL	HLA-B 0801	GP		bind			VMAPRTVLL		HLA-E	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_1_1_s_90	9427624	221 cells at 26 degrees C in the presence of exogenous added peptides: MVDGTLLLL from HLA-E leader sequence which is not capable of binding to HLA-E  in vitro and VMAPRTVLL from HLA-B 0801 which can bind to HLA-E.	bind
29224	1	7344	7	NULL	NULL	0	NULL	HLA-E leader sequence	NULL		does not bind	NULL		MVDGTLLLL		HLA-E	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_currbiol_8_1_1_s_90	9427624	221 cells at 26 degrees C in the presence of exogenous added peptides: MVDGTLLLL from HLA-E leader sequence which is not capable of binding to HLA-E  in vitro and VMAPRTVLL from HLA-B 0801 which can bind to HLA-E.	bind
29225	2	7344	7	NULL	NULL	0	NULL	HLA-B 0801	NULL		binds to	NULL		VMAPRTVLL 		HLA-E	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_8_1_1_s_90	9427624	221 cells at 26 degrees C in the presence of exogenous added peptides: MVDGTLLLL from HLA-E leader sequence which is not capable of binding to HLA-E  in vitro and VMAPRTVLL from HLA-B 0801 which can bind to HLA-E.	bind
26842	1	7345	5	13	NULL	NULL	NULL	HLA-A 0201	GP		bind			leader sequence peptide		HLA-E	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_1_1_s_107	9427624	221 cells transfected with HLA-A 0201, whose leader sequence peptide binds to HLA-E  [25]  .	bind
29226	1	7345	7	NULL	NULL	0	NULL	HLA-A 0201	NULL		binds to	NULL		leader sequence peptide		HLA-E	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_8_1_1_s_107	9427624	221 cells transfected with HLA-A 0201, whose leader sequence peptide binds to HLA-E  [25]  .	bind
26844	1	7346	5	13	NULL	NULL	NULL				bind			ralpha2I domain		collagen type I	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_6_3513_s_277	9920897	229ox peptide inhibits ralpha2I domain binding to collagens type I and IV and to laminin-1.	bind
26845	2	7346	5	13	NULL	NULL	NULL				bind			ralpha2I domain		collagen type IV	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_6_3513_s_277	9920897	229ox peptide inhibits ralpha2I domain binding to collagens type I and IV and to laminin-1.	bind
26846	3	7346	5	13	NULL	NULL	NULL				bind			ralpha2I domain		laminin-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_6_3513_s_277	9920897	229ox peptide inhibits ralpha2I domain binding to collagens type I and IV and to laminin-1.	bind
26847	4	7346	5	13	NULL	NULL	NULL	229ox peptide	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_6_3513_s_277	9920897	229ox peptide inhibits ralpha2I domain binding to collagens type I and IV and to laminin-1.	bind
26848	5	7346	5	13	NULL	NULL	NULL	229ox peptide	GP		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_6_3513_s_277	9920897	229ox peptide inhibits ralpha2I domain binding to collagens type I and IV and to laminin-1.	bind
26849	6	7346	5	13	NULL	NULL	NULL	229ox peptide	GP		inhibit					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_6_3513_s_277	9920897	229ox peptide inhibits ralpha2I domain binding to collagens type I and IV and to laminin-1.	bind
29227	1	7346	7	NULL	NULL	0	NULL		NULL		binds to	NULL		ralpha2I domain		collagen type I	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_6_3513_s_277	9920897	229ox peptide inhibits ralpha2I domain binding to collagens type I and IV and to laminin-1.	bind
29228	2	7346	7	NULL	NULL	0	NULL		NULL		binds to	NULL		ralpha2I domain		collagen type IV	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_6_3513_s_277	9920897	229ox peptide inhibits ralpha2I domain binding to collagens type I and IV and to laminin-1.	bind
29229	3	7346	7	NULL	NULL	0	NULL		NULL		binds to	NULL		ralpha2I domain		laminin-1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_6_3513_s_277	9920897	229ox peptide inhibits ralpha2I domain binding to collagens type I and IV and to laminin-1.	bind
29230	4	7346	7	NULL	NULL	0	NULL	ox peptide	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_6_3513_s_277	9920897	229ox peptide inhibits ralpha2I domain binding to collagens type I and IV and to laminin-1.	bind
29231	5	7346	7	NULL	NULL	0	NULL	ox peptide	NULL		inhibits	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_6_3513_s_277	9920897	229ox peptide inhibits ralpha2I domain binding to collagens type I and IV and to laminin-1.	bind
29232	6	7346	7	NULL	NULL	0	NULL	ox peptide	NULL		inhibits	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_6_3513_s_277	9920897	229ox peptide inhibits ralpha2I domain binding to collagens type I and IV and to laminin-1.	bind
26850	1	7347	5	13	NULL	NULL	NULL	snR10	NucleicAcid		is a type of					small nucleolar RNAs	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_598_s_264	11160879	23       Bagni,C. and Lapeyre,B. (1998) Gar1p binds to the small nucleolar RNAs snR10 and snR30 in vitro through a nontypical RNA binding element.	bind
26851	2	7347	5	13	NULL	NULL	NULL	snR30	NucleicAcid		is a type of					small nucleolar RNAs	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_598_s_264	11160879	23       Bagni,C. and Lapeyre,B. (1998) Gar1p binds to the small nucleolar RNAs snR10 and snR30 in vitro through a nontypical RNA binding element.	bind
26852	3	7347	5	13	NULL	NULL	NULL	Gar1p	GP		bind			nontypical RNA binding element		snR10	NucleicAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_598_s_264	11160879	23       Bagni,C. and Lapeyre,B. (1998) Gar1p binds to the small nucleolar RNAs snR10 and snR30 in vitro through a nontypical RNA binding element.	bind
26853	4	7347	5	13	NULL	NULL	NULL	Gar1p	GP		bind			nontypical RNA binding element		snR30	NucleicAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_598_s_264	11160879	23       Bagni,C. and Lapeyre,B. (1998) Gar1p binds to the small nucleolar RNAs snR10 and snR30 in vitro through a nontypical RNA binding element.	bind
29233	1	7347	7	NULL	NULL	0	NULL	Gar1p	NULL		binds to	NULL				snR10	NULL		nontypical RNA binding element		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_598_s_264	11160879	23       Bagni,C. and Lapeyre,B. (1998) Gar1p binds to the small nucleolar RNAs snR10 and snR30 in vitro through a nontypical RNA binding element.	bind
29234	2	7347	7	NULL	NULL	0	NULL	Gar1p	NULL		binds to	NULL				snR30	NULL		nontypical RNA binding element		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_598_s_264	11160879	23       Bagni,C. and Lapeyre,B. (1998) Gar1p binds to the small nucleolar RNAs snR10 and snR30 in vitro through a nontypical RNA binding element.	bind
29235	3	7347	7	NULL	NULL	0	NULL	snR10	NULL		is a type of	NULL				small nucleolar RNA	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_598_s_264	11160879	23       Bagni,C. and Lapeyre,B. (1998) Gar1p binds to the small nucleolar RNAs snR10 and snR30 in vitro through a nontypical RNA binding element.	bind
29236	4	7347	7	NULL	NULL	0	NULL	snR30	NULL		is a type of	NULL				small nucleolar RNA	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_598_s_264	11160879	23       Bagni,C. and Lapeyre,B. (1998) Gar1p binds to the small nucleolar RNAs snR10 and snR30 in vitro through a nontypical RNA binding element.	bind
26854	1	7348	5	13	NULL	NULL	NULL	Ral	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_899_s_35	11397694	23  Binding to calmodulin enhances GTP binding to Ral 2- to 3-fold.	bind
26855	2	7348	5	13	NULL	NULL	NULL	calmodulin	GP	binding to	enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_899_s_35	11397694	23  Binding to calmodulin enhances GTP binding to Ral 2- to 3-fold.	bind
29237	1	7348	7	NULL	NULL	0	NULL	GTP	NULL		binds	NULL				Ral	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_899_s_35	11397694	23  Binding to calmodulin enhances GTP binding to Ral 2- to 3-fold.	bind
29238	2	7348	7	NULL	NULL	0	NULL	calmodulin	NULL	binding to	enhances	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_899_s_35	11397694	23  Binding to calmodulin enhances GTP binding to Ral 2- to 3-fold.	bind
26856	1	7349	5	13	NULL	NULL	NULL	CD80	GP		bind					CTLA4	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_3_977_s_175	11238045	23  CD80 and CD86 also bind CTLA4, an Ig superfamily member with homology to CD28, which delivers a negative signal to activated T cells.	bind
26857	2	7349	5	13	NULL	NULL	NULL	CD86	GP		bind					CTLA4	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_3_977_s_175	11238045	23  CD80 and CD86 also bind CTLA4, an Ig superfamily member with homology to CD28, which delivers a negative signal to activated T cells.	bind
26858	3	7349	5	13	NULL	NULL	NULL	CTLA4	GP		is a member of					Ig superfamily	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_3_977_s_175	11238045	23  CD80 and CD86 also bind CTLA4, an Ig superfamily member with homology to CD28, which delivers a negative signal to activated T cells.	bind
26859	4	7349	5	13	NULL	NULL	NULL	CTLA4	GP		is homologous to					CD28	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_3_977_s_175	11238045	23  CD80 and CD86 also bind CTLA4, an Ig superfamily member with homology to CD28, which delivers a negative signal to activated T cells.	bind
26860	5	7349	5	13	NULL	NULL	NULL	CTLA4	GP		delivers					T cells	Cell	negative signal to activated			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_3_977_s_175	11238045	23  CD80 and CD86 also bind CTLA4, an Ig superfamily member with homology to CD28, which delivers a negative signal to activated T cells.	bind
29239	1	7349	7	NULL	NULL	0	NULL	CD80	NULL		bind	NULL				CTLA4	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_3_977_s_175	11238045	23  CD80 and CD86 also bind CTLA4, an Ig superfamily member with homology to CD28, which delivers a negative signal to activated T cells.	bind
29240	2	7349	7	NULL	NULL	0	NULL	CD86	NULL		bind	NULL				CTLA4	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_3_977_s_175	11238045	23  CD80 and CD86 also bind CTLA4, an Ig superfamily member with homology to CD28, which delivers a negative signal to activated T cells.	bind
29241	3	7349	7	10	NULL	0	NULL	CTLA4			is a member of					Ig superfamily					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_3_977_s_175	11238045	23  CD80 and CD86 also bind CTLA4, an Ig superfamily member with homology to CD28, which delivers a negative signal to activated T cells.	bind
29242	4	7349	7	NULL	NULL	0	NULL	CTLA4	NULL		is homologous to	NULL				CD28	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_3_977_s_175	11238045	23  CD80 and CD86 also bind CTLA4, an Ig superfamily member with homology to CD28, which delivers a negative signal to activated T cells.	bind
29243	5	7349	7	NULL	NULL	0	NULL	CTLA4	NULL		delivers	NULL				T cells	NULL	negative signal to activated			NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_3_977_s_175	11238045	23  CD80 and CD86 also bind CTLA4, an Ig superfamily member with homology to CD28, which delivers a negative signal to activated T cells.	bind
26861	1	7350	5	13	NULL	NULL	NULL	FK506	Chemical		is more potent than					CsA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_24_2449_s_148	10595959	23  FK506 is 10 to 100 times more potent than CsA. 24  FK506 binds to FK506 binding protein (FKBP), and the FK506/FKBP complex inhibits calcineurin.	bind
26862	2	7350	5	13	NULL	NULL	NULL	FKBP	GP		is					FK506 binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_24_2449_s_148	10595959	23  FK506 is 10 to 100 times more potent than CsA. 24  FK506 binds to FK506 binding protein (FKBP), and the FK506/FKBP complex inhibits calcineurin.	bind
26863	3	7350	5	13	NULL	NULL	NULL	FK506	Chemical		bind					FKBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_24_2449_s_148	10595959	23  FK506 is 10 to 100 times more potent than CsA. 24  FK506 binds to FK506 binding protein (FKBP), and the FK506/FKBP complex inhibits calcineurin.	bind
26864	4	7350	5	13	NULL	NULL	NULL	FK506/FKBP complex	GP		inhibit					calcineurin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_24_2449_s_148	10595959	23  FK506 is 10 to 100 times more potent than CsA. 24  FK506 binds to FK506 binding protein (FKBP), and the FK506/FKBP complex inhibits calcineurin.	bind
29244	1	7350	7	NULL	NULL	0	NULL	FK506	NULL		is more potent than	NULL				CsA	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_100_24_2449_s_148	10595959	23  FK506 is 10 to 100 times more potent than CsA. 24  FK506 binds to FK506 binding protein (FKBP), and the FK506/FKBP complex inhibits calcineurin.	bind
29245	2	7350	7	NULL	NULL	0	NULL	 FK506	NULL		binds	NULL				FKBP	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_100_24_2449_s_148	10595959	23  FK506 is 10 to 100 times more potent than CsA. 24  FK506 binds to FK506 binding protein (FKBP), and the FK506/FKBP complex inhibits calcineurin.	bind
29246	3	7350	7	NULL	NULL	0	NULL	FK506/FKBP complex	NULL		inhibits	NULL				calcineurin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_100_24_2449_s_148	10595959	23  FK506 is 10 to 100 times more potent than CsA. 24  FK506 binds to FK506 binding protein (FKBP), and the FK506/FKBP complex inhibits calcineurin.	bind
29247	4	7350	7	NULL	NULL	0	NULL	FKBP	NULL		is	NULL				FK506 binding protein	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_100_24_2449_s_148	10595959	23  FK506 is 10 to 100 times more potent than CsA. 24  FK506 binds to FK506 binding protein (FKBP), and the FK506/FKBP complex inhibits calcineurin.	bind
26865	2	7351	5	13	NULL	NULL	NULL	IL-13Ralpha2	GP		is inhibitor of		potent			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_162_5_1475_s_105	12707030	23  IL-13Ralpha2 acts as a potent inhibitor of IL-13 binding to its cell surface receptor leading to the initial suggestion 24  and later demonstration 26,27 that it modulates the effects of IL-13  in vivo.	bind
26866	1	7351	5	13	NULL	NULL	NULL	IL-13	GP		bind					cell surface receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_162_5_1475_s_105	12707030	23  IL-13Ralpha2 acts as a potent inhibitor of IL-13 binding to its cell surface receptor leading to the initial suggestion 24  and later demonstration 26,27 that it modulates the effects of IL-13  in vivo.	bind
26867	3	7351	5	13	NULL	NULL	NULL	IL-13Ralpha2	GP		modulates					IL-13	GP	effects of			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_amjpathol_162_5_1475_s_105	12707030	23  IL-13Ralpha2 acts as a potent inhibitor of IL-13 binding to its cell surface receptor leading to the initial suggestion 24  and later demonstration 26,27 that it modulates the effects of IL-13  in vivo.	bind
29248	1	7351	7	NULL	NULL	0	NULL	IL-13	NULL		binds to	NULL				cell surface receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_162_5_1475_s_105	12707030	23  IL-13Ralpha2 acts as a potent inhibitor of IL-13 binding to its cell surface receptor leading to the initial suggestion 24  and later demonstration 26,27 that it modulates the effects of IL-13  in vivo.	bind
29249	2	7351	7	NULL	NULL	0	NULL	IL-13Ralpha2	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_162_5_1475_s_105	12707030	23  IL-13Ralpha2 acts as a potent inhibitor of IL-13 binding to its cell surface receptor leading to the initial suggestion 24  and later demonstration 26,27 that it modulates the effects of IL-13  in vivo.	bind
29250	3	7351	7	NULL	NULL	0	NULL	IL-13Ralpha2	NULL		modulates	NULL				IL-13	NULL	effects of			NULL	in vivo	0	NULL	NULL	NULL	gw60_amjpathol_162_5_1475_s_105	12707030	23  IL-13Ralpha2 acts as a potent inhibitor of IL-13 binding to its cell surface receptor leading to the initial suggestion 24  and later demonstration 26,27 that it modulates the effects of IL-13  in vivo.	bind
26868	1	7352	5	13	NULL	NULL	NULL	PAI-1	GP		is inhibitor of					serpin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_6_1095_s_45	7586221	23  PAI-1 is a serpin inhibitor that endogenously binds and inactivates plasminogen activators such as TPA and UPA.	bind
26869	2	7352	5	13	NULL	NULL	NULL	TPA	GP		is a type of					plasminogen activator	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_6_1095_s_45	7586221	23  PAI-1 is a serpin inhibitor that endogenously binds and inactivates plasminogen activators such as TPA and UPA.	bind
26870	3	7352	5	13	NULL	NULL	NULL	UPA	GP		is a type of					plasminogen activator	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_6_1095_s_45	7586221	23  PAI-1 is a serpin inhibitor that endogenously binds and inactivates plasminogen activators such as TPA and UPA.	bind
26871	4	7352	5	13	NULL	NULL	NULL	PAI-1	GP		bind		endogenously			TPA	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_6_1095_s_45	7586221	23  PAI-1 is a serpin inhibitor that endogenously binds and inactivates plasminogen activators such as TPA and UPA.	bind
26872	5	7352	5	13	NULL	NULL	NULL	PAI-1	GP		inactivates		endogenously			TPA	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_6_1095_s_45	7586221	23  PAI-1 is a serpin inhibitor that endogenously binds and inactivates plasminogen activators such as TPA and UPA.	bind
26873	6	7352	5	13	NULL	NULL	NULL	PAI-1	GP		bind		endogenously			UPA	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_6_1095_s_45	7586221	23  PAI-1 is a serpin inhibitor that endogenously binds and inactivates plasminogen activators such as TPA and UPA.	bind
26874	7	7352	5	13	NULL	NULL	NULL	PAI-1	GP		inactivates		endogenously			UPA	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_6_1095_s_45	7586221	23  PAI-1 is a serpin inhibitor that endogenously binds and inactivates plasminogen activators such as TPA and UPA.	bind
29251	1	7352	7	NULL	NULL	0	NULL	PAI-1	NULL		is a type of	NULL				serpin inhibitor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_77_6_1095_s_45	7586221	23  PAI-1 is a serpin inhibitor that endogenously binds and inactivates plasminogen activators such as TPA and UPA.	bind
29252	2	7352	7	NULL	NULL	0	NULL	PAI-1	NULL		binds	NULL	endogenously			TPA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_6_1095_s_45	7586221	23  PAI-1 is a serpin inhibitor that endogenously binds and inactivates plasminogen activators such as TPA and UPA.	bind
29253	3	7352	7	NULL	NULL	0	NULL	PAI-1	NULL		binds 	NULL	endogenously			UPA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_6_1095_s_45	7586221	23  PAI-1 is a serpin inhibitor that endogenously binds and inactivates plasminogen activators such as TPA and UPA.	bind
29254	4	7352	7	10	NULL	0	NULL	PAI-1			inactivates		endogenously			TPA					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_6_1095_s_45	7586221	23  PAI-1 is a serpin inhibitor that endogenously binds and inactivates plasminogen activators such as TPA and UPA.	bind
29255	5	7352	7	10	NULL	0	NULL	PAI-1			inactivates		endogenously			UPA					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_6_1095_s_45	7586221	23  PAI-1 is a serpin inhibitor that endogenously binds and inactivates plasminogen activators such as TPA and UPA.	bind
29256	6	7352	7	NULL	NULL	0	NULL	TPA	NULL		is a type of	NULL				plasminogen activator	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_77_6_1095_s_45	7586221	23  PAI-1 is a serpin inhibitor that endogenously binds and inactivates plasminogen activators such as TPA and UPA.	bind
29257	7	7352	7	NULL	NULL	0	NULL	uPA	NULL		is a type of	NULL				plasminogen activator	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_77_6_1095_s_45	7586221	23  PAI-1 is a serpin inhibitor that endogenously binds and inactivates plasminogen activators such as TPA and UPA.	bind
26875	1	7353	5	13	NULL	NULL	NULL	KDR	GP		bind					bFGF	GP				NULL	KS cells	NULL	NULL	NULL	NULL	gw60_amjpathol_156_4_1381_s_119	10751362	23  Supernatants from KS cells, 27  which contain bFGF and VEGF, and Tat, which binds the VEGF receptor KDR, 28 strongly induce angiogenesis.	bind
26876	2	7353	5	13	NULL	NULL	NULL	KDR	GP		bind					VEGF	GP				NULL	KS cells	NULL	NULL	NULL	NULL	gw60_amjpathol_156_4_1381_s_119	10751362	23  Supernatants from KS cells, 27  which contain bFGF and VEGF, and Tat, which binds the VEGF receptor KDR, 28 strongly induce angiogenesis.	bind
26918	3	7353	5	13	NULL	NULL	NULL	KDR	GP		is a type of					VEGF receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_4_1381_s_119	10751362	23  Supernatants from KS cells, 27  which contain bFGF and VEGF, and Tat, which binds the VEGF receptor KDR, 28 strongly induce angiogenesis.	bind
26919	4	7353	5	13	NULL	NULL	NULL	Tat	GP		bind					KDR	GP				NULL	KS cells	NULL	NULL	NULL	NULL	gw60_amjpathol_156_4_1381_s_119	10751362	23  Supernatants from KS cells, 27  which contain bFGF and VEGF, and Tat, which binds the VEGF receptor KDR, 28 strongly induce angiogenesis.	bind
27039	5	7353	5	13	NULL	NULL	NULL	statement 1	Process		induces		strongly			angiogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_4_1381_s_119	10751362	23  Supernatants from KS cells, 27  which contain bFGF and VEGF, and Tat, which binds the VEGF receptor KDR, 28 strongly induce angiogenesis.	bind
27040	6	7353	5	13	NULL	NULL	NULL	statement 2	Process		induces		strongly			angiogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_4_1381_s_119	10751362	23  Supernatants from KS cells, 27  which contain bFGF and VEGF, and Tat, which binds the VEGF receptor KDR, 28 strongly induce angiogenesis.	bind
27041	7	7353	5	13	NULL	NULL	NULL	statement 4	Process		induces		strongly			angiogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_4_1381_s_119	10751362	23  Supernatants from KS cells, 27  which contain bFGF and VEGF, and Tat, which binds the VEGF receptor KDR, 28 strongly induce angiogenesis.	bind
29258	1	7353	7	NULL	NULL	0	NULL	bFGF	NULL		binds	NULL				KDR	NULL				NULL	KS cells	NULL	NULL	NULL	NULL	gw60_amjpathol_156_4_1381_s_119	10751362	23  Supernatants from KS cells, 27  which contain bFGF and VEGF, and Tat, which binds the VEGF receptor KDR, 28 strongly induce angiogenesis.	bind
29259	2	7353	7	NULL	NULL	0	NULL	VEGF	NULL		binds	NULL				KDR	NULL				NULL	KS cells	NULL	NULL	NULL	NULL	gw60_amjpathol_156_4_1381_s_119	10751362	23  Supernatants from KS cells, 27  which contain bFGF and VEGF, and Tat, which binds the VEGF receptor KDR, 28 strongly induce angiogenesis.	bind
29260	3	7353	7	NULL	NULL	0	NULL	Tat	NULL		binds	NULL				KDR	NULL				NULL	KS cells	NULL	NULL	NULL	NULL	gw60_amjpathol_156_4_1381_s_119	10751362	23  Supernatants from KS cells, 27  which contain bFGF and VEGF, and Tat, which binds the VEGF receptor KDR, 28 strongly induce angiogenesis.	bind
29261	4	7353	7	NULL	NULL	0	NULL	statement 1	NULL		induce	NULL	strongly			angiogenesis	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_4_1381_s_119	10751362	23  Supernatants from KS cells, 27  which contain bFGF and VEGF, and Tat, which binds the VEGF receptor KDR, 28 strongly induce angiogenesis.	bind
29262	5	7353	7	NULL	NULL	0	NULL	statement 2	NULL		induce	NULL	strongly			angiogenesis	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_4_1381_s_119	10751362	23  Supernatants from KS cells, 27  which contain bFGF and VEGF, and Tat, which binds the VEGF receptor KDR, 28 strongly induce angiogenesis.	bind
29263	6	7353	7	NULL	NULL	0	NULL	statement 3	NULL		induce	NULL	strongly			angiogenesis	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_4_1381_s_119	10751362	23  Supernatants from KS cells, 27  which contain bFGF and VEGF, and Tat, which binds the VEGF receptor KDR, 28 strongly induce angiogenesis.	bind
29265	7	7353	7	NULL	NULL	0	NULL	KDR	NULL		is a type of	NULL				VEGF receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_4_1381_s_119	10751362	23  Supernatants from KS cells, 27  which contain bFGF and VEGF, and Tat, which binds the VEGF receptor KDR, 28 strongly induce angiogenesis.	bind
27042	1	7354	5	13	NULL	NULL	NULL	FGF ligand	GP	binding of	requires							different	structural motifs within HS chains		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_185_s_17	11786412	23  The HS-binding regions of FGF ligand and RTK require different structural motifs within the HS chains for binding.	bind
27044	3	7354	5	13	NULL	NULL	NULL	RTK	GP	binding of	requires								structural motifs within HS chains		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_185_s_17	11786412	23  The HS-binding regions of FGF ligand and RTK require different structural motifs within the HS chains for binding.	bind
29271	1	7354	7	10	NULL	0	NULL	FGF ligand 	NULL	binding of	requires	NULL					NULL		structural motifs within the HS chains		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_185_s_17	11786412	23  The HS-binding regions of FGF ligand and RTK require different structural motifs within the HS chains for binding.	bind
29272	2	7354	7	10	NULL	0	NULL	RTK	NULL	binding of	requires	NULL					NULL		structural motifs within the HS chains		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_185_s_17	11786412	23  The HS-binding regions of FGF ligand and RTK require different structural motifs within the HS chains for binding.	bind
27047	1	7356	5	13	NULL	NULL	NULL	Src	GP		bind					PDGF beta-receptor	GP	autophosphorylated	phosphotyrosine residue 579		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_1_12_s_34	10400906	23 24  Activation occurs by the binding of  Src to the autophosphorylated PDGF beta-receptor at phosphotyrosine residues 579 and 581.	bind
27048	2	7356	5	13	NULL	NULL	NULL	statement 1	Process		leads to					activation	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_1_12_s_34	10400906	23 24  Activation occurs by the binding of  Src to the autophosphorylated PDGF beta-receptor at phosphotyrosine residues 579 and 581.	bind
27049	3	7356	5	13	NULL	NULL	NULL	Src	GP		bind					PDGF beta-receptor	GP	autophosphorylated	phosphotyrosine residue 581		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_1_12_s_34	10400906	23 24  Activation occurs by the binding of  Src to the autophosphorylated PDGF beta-receptor at phosphotyrosine residues 579 and 581.	bind
27050	4	7356	5	13	NULL	NULL	NULL	statement 3	Process		leads to					activation	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_1_12_s_34	10400906	23 24  Activation occurs by the binding of  Src to the autophosphorylated PDGF beta-receptor at phosphotyrosine residues 579 and 581.	bind
29344	1	7356	7	NULL	NULL	0	NULL	Src	NULL		binds	NULL				PDGF beta-receptor	NULL	autophosphorylated	phosphotyrosine residues 579 		NULL		0	NULL	NULL	NULL	gw60_circulationres_85_1_12_s_34	10400906	23 24  Activation occurs by the binding of  Src to the autophosphorylated PDGF beta-receptor at phosphotyrosine residues 579 and 581.	bind
29345	2	7356	7	NULL	NULL	0	NULL	Src	NULL		binds	NULL				PDGF beta-receptor	NULL	autophosphorylated	phosphotyrosine residues 581		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_1_12_s_34	10400906	23 24  Activation occurs by the binding of  Src to the autophosphorylated PDGF beta-receptor at phosphotyrosine residues 579 and 581.	bind
29346	3	7356	7	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				activation	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_85_1_12_s_34	10400906	23 24  Activation occurs by the binding of  Src to the autophosphorylated PDGF beta-receptor at phosphotyrosine residues 579 and 581.	bind
29347	4	7356	7	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				activation	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_85_1_12_s_34	10400906	23 24  Activation occurs by the binding of  Src to the autophosphorylated PDGF beta-receptor at phosphotyrosine residues 579 and 581.	bind
27051	1	7357	5	13	NULL	NULL	NULL	prothrombin	GP		bind		may			VLDLs	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_1_33_s_32	9445253	23 24 25  It is still unknown whether vitamin K - dependent proteins interact with TGRLP in vivo, although prothrombin and factor Xa may bind to VLDLs in vitro, partially through a calcium-dependent association.	bind
27052	2	7357	5	13	NULL	NULL	NULL	factor Xa	GP		bind		may			VLDLs	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_1_33_s_32	9445253	23 24 25  It is still unknown whether vitamin K - dependent proteins interact with TGRLP in vivo, although prothrombin and factor Xa may bind to VLDLs in vitro, partially through a calcium-dependent association.	bind
27053	3	7357	5	13	NULL	NULL	NULL	statement 1	Process		is dependent on		partially			calcium	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_1_33_s_32	9445253	23 24 25  It is still unknown whether vitamin K - dependent proteins interact with TGRLP in vivo, although prothrombin and factor Xa may bind to VLDLs in vitro, partially through a calcium-dependent association.	bind
27054	4	7357	5	13	NULL	NULL	NULL	statement 2	Process		is dependent on		partially			calcium	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_1_33_s_32	9445253	23 24 25  It is still unknown whether vitamin K - dependent proteins interact with TGRLP in vivo, although prothrombin and factor Xa may bind to VLDLs in vitro, partially through a calcium-dependent association.	bind
29348	1	7357	7	NULL	NULL	0	NULL	prothrombin	NULL		bind	NULL	may			VLDL	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_1_33_s_32	9445253	23 24 25  It is still unknown whether vitamin K - dependent proteins interact with TGRLP in vivo, although prothrombin and factor Xa may bind to VLDLs in vitro, partially through a calcium-dependent association.	bind
29349	2	7357	7	NULL	NULL	0	NULL	factor Xa	NULL		bind	NULL	may			VLDL	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_1_33_s_32	9445253	23 24 25  It is still unknown whether vitamin K - dependent proteins interact with TGRLP in vivo, although prothrombin and factor Xa may bind to VLDLs in vitro, partially through a calcium-dependent association.	bind
29350	3	7357	7	10	NULL	0	NULL	statement 1	NULL		is dependent on	NULL	partially			calcium	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_1_33_s_32	9445253	23 24 25  It is still unknown whether vitamin K - dependent proteins interact with TGRLP in vivo, although prothrombin and factor Xa may bind to VLDLs in vitro, partially through a calcium-dependent association.	bind
29351	4	7357	7	10	NULL	0	NULL	statement 2	NULL		is dependent on	NULL	partially			calcium	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_1_33_s_32	9445253	23 24 25  It is still unknown whether vitamin K - dependent proteins interact with TGRLP in vivo, although prothrombin and factor Xa may bind to VLDLs in vitro, partially through a calcium-dependent association.	bind
27056	1	7360	5	13	NULL	NULL	NULL	HDLs	GP	apoA-II - enriched	bind					SR-BI	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_4_638_s_91	11950703	23 However, although apoA-II - enriched HDLs bind to human SR-BI with higher affinity than apoA-I - rich HDLs, they display a lower capacity to deliver cholesteryl esters to human adrenal cells.	bind
27057	2	7360	5	13	NULL	NULL	NULL	HDLs	GP	apoA-I - rich	bind					SR-BI	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_4_638_s_91	11950703	23 However, although apoA-II - enriched HDLs bind to human SR-BI with higher affinity than apoA-I - rich HDLs, they display a lower capacity to deliver cholesteryl esters to human adrenal cells.	bind
27058	3	7360	5	13	NULL	NULL	NULL	statement 1	Process		has high affinity than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_4_638_s_91	11950703	23 However, although apoA-II - enriched HDLs bind to human SR-BI with higher affinity than apoA-I - rich HDLs, they display a lower capacity to deliver cholesteryl esters to human adrenal cells.	bind
27067	4	7360	5	13	NULL	NULL	NULL	cholesteryl esters	Chemical		is delivered to					adrenal cells	Cell	human			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_4_638_s_91	11950703	23 However, although apoA-II - enriched HDLs bind to human SR-BI with higher affinity than apoA-I - rich HDLs, they display a lower capacity to deliver cholesteryl esters to human adrenal cells.	bind
27070	5	7360	5	13	NULL	NULL	NULL	HDLs	GP	apoA-II - enriched	display					statement 4	Process	lower capacity to			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_4_638_s_91	11950703	23 However, although apoA-II - enriched HDLs bind to human SR-BI with higher affinity than apoA-I - rich HDLs, they display a lower capacity to deliver cholesteryl esters to human adrenal cells.	bind
29353	1	7360	7	NULL	NULL	0	NULL	HDLs	NULL	apoA-II - enriched	binds to	NULL				SR-BI 	NULL	human			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_4_638_s_91	11950703	23 However, although apoA-II - enriched HDLs bind to human SR-BI with higher affinity than apoA-I - rich HDLs, they display a lower capacity to deliver cholesteryl esters to human adrenal cells.	bind
29354	2	7360	7	NULL	NULL	0	NULL	HDLs	NULL	apoA-I - rich	binds to	NULL				SR-BI	NULL	human			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_4_638_s_91	11950703	23 However, although apoA-II - enriched HDLs bind to human SR-BI with higher affinity than apoA-I - rich HDLs, they display a lower capacity to deliver cholesteryl esters to human adrenal cells.	bind
29355	3	7360	7	NULL	NULL	0	NULL	statement 1	NULL		higher affinity than	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_4_638_s_91	11950703	23 However, although apoA-II - enriched HDLs bind to human SR-BI with higher affinity than apoA-I - rich HDLs, they display a lower capacity to deliver cholesteryl esters to human adrenal cells.	bind
29357	4	7360	7	NULL	NULL	0	NULL	 cholesteryl esters	NULL		is delivered to	NULL				adrenal cells	NULL	human			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_4_638_s_91	11950703	23 However, although apoA-II - enriched HDLs bind to human SR-BI with higher affinity than apoA-I - rich HDLs, they display a lower capacity to deliver cholesteryl esters to human adrenal cells.	bind
29358	5	7360	7	NULL	NULL	0	NULL	HDLs	NULL	apoA-II - enriched	displays 	NULL				statement 4	NULL	a lower capacity to			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_4_638_s_91	11950703	23 However, although apoA-II - enriched HDLs bind to human SR-BI with higher affinity than apoA-I - rich HDLs, they display a lower capacity to deliver cholesteryl esters to human adrenal cells.	bind
29359	1	7361	7	NULL	NULL	0	NULL	HSP90 	NULL		binds to	NULL				PM-eNOS	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_959_s_23	16627819	23 Interestingly, the authors also observed that there was significantly more HSP90 (but not caveolin-1) bound to the PM-eNOS versus the Golgi-eNOS.	bind
29360	2	7361	7	NULL	NULL	0	NULL	HSP90	NULL		binds to	NULL				Golgi-eNOS	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_959_s_23	16627819	23 Interestingly, the authors also observed that there was significantly more HSP90 (but not caveolin-1) bound to the PM-eNOS versus the Golgi-eNOS.	bind
29361	3	7361	7	NULL	NULL	0	NULL	caveolin-1	NULL		does not bind	NULL				PM-eNOS	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_959_s_23	16627819	23 Interestingly, the authors also observed that there was significantly more HSP90 (but not caveolin-1) bound to the PM-eNOS versus the Golgi-eNOS.	bind
29362	4	7361	7	NULL	NULL	0	NULL	caveolin-1	NULL		does not bind	NULL				Golgi-eNOS	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_959_s_23	16627819	23 Interestingly, the authors also observed that there was significantly more HSP90 (but not caveolin-1) bound to the PM-eNOS versus the Golgi-eNOS.	bind
27089	1	7362	5	13	NULL	NULL	NULL	LDL receptor	GP		contains									SRE in promoter	NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_24_3104_s_24	12473559	23 LDL receptor, like other genes involved in lipid metabolism, contains the consensus sterol regulatory elements (SRE) in the promoter, allowing its regulation through SRE-1 binding proteins (SREBPs).	bind
27090	2	7362	5	13	NULL	NULL	NULL	SRE	GP		is					sterol regulatory elements	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_24_3104_s_24	12473559	23 LDL receptor, like other genes involved in lipid metabolism, contains the consensus sterol regulatory elements (SRE) in the promoter, allowing its regulation through SRE-1 binding proteins (SREBPs).	bind
27091	3	7362	5	13	NULL	NULL	NULL	statement 1	GP		allows					SREBPs	GP	regulation through			NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_24_3104_s_24	12473559	23 LDL receptor, like other genes involved in lipid metabolism, contains the consensus sterol regulatory elements (SRE) in the promoter, allowing its regulation through SRE-1 binding proteins (SREBPs).	bind
27092	4	7362	5	13	NULL	NULL	NULL	SREBPs	GP		is					SRE-1 binding proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_24_3104_s_24	12473559	23 LDL receptor, like other genes involved in lipid metabolism, contains the consensus sterol regulatory elements (SRE) in the promoter, allowing its regulation through SRE-1 binding proteins (SREBPs).	bind
29363	1	7362	7	NULL	NULL	0	NULL	LDL receptor gene	NULL		is involved in	NULL				lipid metabolism	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_24_3104_s_24	12473559	23 LDL receptor, like other genes involved in lipid metabolism, contains the consensus sterol regulatory elements (SRE) in the promoter, allowing its regulation through SRE-1 binding proteins (SREBPs).	bind
29364	2	7362	7	NULL	NULL	0	NULL	LDL receptor gene	NULL		contains	NULL					NULL	consensus		SRE in the promoter	NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_24_3104_s_24	12473559	23 LDL receptor, like other genes involved in lipid metabolism, contains the consensus sterol regulatory elements (SRE) in the promoter, allowing its regulation through SRE-1 binding proteins (SREBPs).	bind
29365	3	7362	7	NULL	NULL	0	NULL	LDL receptor gene	NULL		regulates through	NULL				SREBPs	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_24_3104_s_24	12473559	23 LDL receptor, like other genes involved in lipid metabolism, contains the consensus sterol regulatory elements (SRE) in the promoter, allowing its regulation through SRE-1 binding proteins (SREBPs).	bind
29366	4	7362	7	NULL	NULL	0	NULL	SRE	NULL		is	NULL				sterol regulatory elements	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_24_3104_s_24	12473559	23 LDL receptor, like other genes involved in lipid metabolism, contains the consensus sterol regulatory elements (SRE) in the promoter, allowing its regulation through SRE-1 binding proteins (SREBPs).	bind
29367	5	7362	7	NULL	NULL	0	NULL	SREBPs	NULL		is	NULL				SRE-1 binding proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_24_3104_s_24	12473559	23 LDL receptor, like other genes involved in lipid metabolism, contains the consensus sterol regulatory elements (SRE) in the promoter, allowing its regulation through SRE-1 binding proteins (SREBPs).	bind
27093	1	7363	5	13	NULL	NULL	NULL	LXR	GP		is a type of					nuclear hormone receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_116	15178557	23 LXR is a nuclear hormone receptor that binds oxysterols and activates its target genes, such as  CYP7A encoding the rate-limiting enzyme in the conversion of cholesterol to bile acids by dimerizing with retinoid X receptor (RXR).	bind
27094	2	7363	5	13	NULL	NULL	NULL	LXR	GP		bind					oxysterols	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_116	15178557	23 LXR is a nuclear hormone receptor that binds oxysterols and activates its target genes, such as  CYP7A encoding the rate-limiting enzyme in the conversion of cholesterol to bile acids by dimerizing with retinoid X receptor (RXR).	bind
27095	3	7363	5	13	NULL	NULL	NULL	statement 2	Process		activates					CYP7A	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_116	15178557	23 LXR is a nuclear hormone receptor that binds oxysterols and activates its target genes, such as  CYP7A encoding the rate-limiting enzyme in the conversion of cholesterol to bile acids by dimerizing with retinoid X receptor (RXR).	bind
27096	4	7363	5	13	NULL	NULL	NULL	CYP7A	GP		is a type of					LXR target genes	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_116	15178557	23 LXR is a nuclear hormone receptor that binds oxysterols and activates its target genes, such as  CYP7A encoding the rate-limiting enzyme in the conversion of cholesterol to bile acids by dimerizing with retinoid X receptor (RXR).	bind
27097	5	7363	5	13	NULL	NULL	NULL	cholesterol	Chemical		is converted to					bile acids	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_116	15178557	23 LXR is a nuclear hormone receptor that binds oxysterols and activates its target genes, such as  CYP7A encoding the rate-limiting enzyme in the conversion of cholesterol to bile acids by dimerizing with retinoid X receptor (RXR).	bind
27098	6	7363	5	13	NULL	NULL	NULL	LXR	GP		dimerizes with					RXR	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_116	15178557	23 LXR is a nuclear hormone receptor that binds oxysterols and activates its target genes, such as  CYP7A encoding the rate-limiting enzyme in the conversion of cholesterol to bile acids by dimerizing with retinoid X receptor (RXR).	bind
27099	7	7363	5	13	NULL	NULL	NULL	RXR	GP		is					retinoid X receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_116	15178557	23 LXR is a nuclear hormone receptor that binds oxysterols and activates its target genes, such as  CYP7A encoding the rate-limiting enzyme in the conversion of cholesterol to bile acids by dimerizing with retinoid X receptor (RXR).	bind
27100	8	7363	5	13	NULL	NULL	NULL	CYP7A	GP		encodes					rate-limiting enzyme	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_116	15178557	23 LXR is a nuclear hormone receptor that binds oxysterols and activates its target genes, such as  CYP7A encoding the rate-limiting enzyme in the conversion of cholesterol to bile acids by dimerizing with retinoid X receptor (RXR).	bind
27101	9	7363	5	13	NULL	NULL	NULL	statement 8	Process		plays a role in					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_116	15178557	23 LXR is a nuclear hormone receptor that binds oxysterols and activates its target genes, such as  CYP7A encoding the rate-limiting enzyme in the conversion of cholesterol to bile acids by dimerizing with retinoid X receptor (RXR).	bind
29368	1	7363	7	NULL	NULL	0	NULL	LXR	NULL		binds	NULL				oxysterols	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_116	15178557	23 LXR is a nuclear hormone receptor that binds oxysterols and activates its target genes, such as  CYP7A encoding the rate-limiting enzyme in the conversion of cholesterol to bile acids by dimerizing with retinoid X receptor (RXR).	bind
29369	2	7363	7	NULL	NULL	0	NULL	LXR	NULL		activates	NULL				CYP7A genes	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_116	15178557	23 LXR is a nuclear hormone receptor that binds oxysterols and activates its target genes, such as  CYP7A encoding the rate-limiting enzyme in the conversion of cholesterol to bile acids by dimerizing with retinoid X receptor (RXR).	bind
29370	3	7363	7	NULL	NULL	0	NULL	CYP7A	NULL		encodes	NULL				rate-limiting enzyme	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_116	15178557	23 LXR is a nuclear hormone receptor that binds oxysterols and activates its target genes, such as  CYP7A encoding the rate-limiting enzyme in the conversion of cholesterol to bile acids by dimerizing with retinoid X receptor (RXR).	bind
29371	4	7363	7	NULL	NULL	0	NULL	cholesterol	NULL		dimerizes with	NULL				RXR	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_116	15178557	23 LXR is a nuclear hormone receptor that binds oxysterols and activates its target genes, such as  CYP7A encoding the rate-limiting enzyme in the conversion of cholesterol to bile acids by dimerizing with retinoid X receptor (RXR).	bind
29372	5	7363	7	NULL	NULL	0	NULL	cholesterol	NULL		converts to	NULL				bile acids	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_116	15178557	23 LXR is a nuclear hormone receptor that binds oxysterols and activates its target genes, such as  CYP7A encoding the rate-limiting enzyme in the conversion of cholesterol to bile acids by dimerizing with retinoid X receptor (RXR).	bind
29373	6	7363	7	NULL	NULL	0	NULL	rate-limiting enzyme	NULL		is involved in	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_116	15178557	23 LXR is a nuclear hormone receptor that binds oxysterols and activates its target genes, such as  CYP7A encoding the rate-limiting enzyme in the conversion of cholesterol to bile acids by dimerizing with retinoid X receptor (RXR).	bind
29374	7	7363	7	NULL	NULL	0	NULL	LXR	NULL		is a type of	NULL				nuclear hormone receptor	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_116	15178557	23 LXR is a nuclear hormone receptor that binds oxysterols and activates its target genes, such as  CYP7A encoding the rate-limiting enzyme in the conversion of cholesterol to bile acids by dimerizing with retinoid X receptor (RXR).	bind
29375	8	7363	7	NULL	NULL	0	NULL	RXR	NULL		is	NULL				retinoid X receptor	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_116	15178557	23 LXR is a nuclear hormone receptor that binds oxysterols and activates its target genes, such as  CYP7A encoding the rate-limiting enzyme in the conversion of cholesterol to bile acids by dimerizing with retinoid X receptor (RXR).	bind
27140	1	7364	5	13	NULL	NULL	NULL	apoA-I	GP		bind		likely			PS	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_38	12738681	23 The authors suggested that apoA-I is likely bound to phosphatidylserine (PS) that is presented to the exofacial leaflet by the "`floppase"` activity of ABCA1 because PS levels on the exofacial leaflet are increased by ABCA1 expression.	bind
27141	2	7364	5	13	NULL	NULL	NULL	PS	Chemical		is					phosphatidylserine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_38	12738681	23 The authors suggested that apoA-I is likely bound to phosphatidylserine (PS) that is presented to the exofacial leaflet by the "`floppase"` activity of ABCA1 because PS levels on the exofacial leaflet are increased by ABCA1 expression.	bind
27142	3	7364	5	13	NULL	NULL	NULL	PS	Chemical		is presented to					exofacial leaflet					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_38	12738681	23 The authors suggested that apoA-I is likely bound to phosphatidylserine (PS) that is presented to the exofacial leaflet by the "`floppase"` activity of ABCA1 because PS levels on the exofacial leaflet are increased by ABCA1 expression.	bind
27143	4	7364	5	13	NULL	NULL	NULL	ABCA1	GP		exhibits					floppase activity	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_38	12738681	23 The authors suggested that apoA-I is likely bound to phosphatidylserine (PS) that is presented to the exofacial leaflet by the "`floppase"` activity of ABCA1 because PS levels on the exofacial leaflet are increased by ABCA1 expression.	bind
27144	5	7364	5	13	NULL	NULL	NULL	PS	Chemical	levels of	is increased by					ABCA1	GP	expression of			NULL	exofacial leaflet	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_38	12738681	23 The authors suggested that apoA-I is likely bound to phosphatidylserine (PS) that is presented to the exofacial leaflet by the "`floppase"` activity of ABCA1 because PS levels on the exofacial leaflet are increased by ABCA1 expression.	bind
46589	6	7364	5	13	NULL	NULL	NULL	statement 3	Process		occurs by					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_38	12738681	23 The authors suggested that apoA-I is likely bound to phosphatidylserine (PS) that is presented to the exofacial leaflet by the "`floppase"` activity of ABCA1 because PS levels on the exofacial leaflet are increased by ABCA1 expression.	bind
29376	1	7364	7	NULL	NULL	0	NULL	apoA-I	NULL		bind	NULL				PS	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_38	12738681	23 The authors suggested that apoA-I is likely bound to phosphatidylserine (PS) that is presented to the exofacial leaflet by the "`floppase"` activity of ABCA1 because PS levels on the exofacial leaflet are increased by ABCA1 expression.	bind
29377	2	7364	7	10	NULL	0	NULL	PS			is presented to					 exofacial leaflet					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_38	12738681	23 The authors suggested that apoA-I is likely bound to phosphatidylserine (PS) that is presented to the exofacial leaflet by the "`floppase"` activity of ABCA1 because PS levels on the exofacial leaflet are increased by ABCA1 expression.	bind
29378	3	7364	7	10	NULL	0	NULL	ABCA1	NULL		exhibits	NULL				floppase activity	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_38	12738681	23 The authors suggested that apoA-I is likely bound to phosphatidylserine (PS) that is presented to the exofacial leaflet by the "`floppase"` activity of ABCA1 because PS levels on the exofacial leaflet are increased by ABCA1 expression.	bind
29379	4	7364	7	10	NULL	0	NULL	ABCA1 expression			increase					PS 		levels of			NULL	exofacial leaflet	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_38	12738681	23 The authors suggested that apoA-I is likely bound to phosphatidylserine (PS) that is presented to the exofacial leaflet by the "`floppase"` activity of ABCA1 because PS levels on the exofacial leaflet are increased by ABCA1 expression.	bind
29380	5	7364	7	NULL	NULL	0	NULL	statement 3	NULL		because of	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_38	12738681	23 The authors suggested that apoA-I is likely bound to phosphatidylserine (PS) that is presented to the exofacial leaflet by the "`floppase"` activity of ABCA1 because PS levels on the exofacial leaflet are increased by ABCA1 expression.	bind
29381	6	7364	7	NULL	NULL	0	NULL	PS	NULL		is	NULL				phosphatidylserine	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_38	12738681	23 The authors suggested that apoA-I is likely bound to phosphatidylserine (PS) that is presented to the exofacial leaflet by the "`floppase"` activity of ABCA1 because PS levels on the exofacial leaflet are increased by ABCA1 expression.	bind
46590	7	7364	7	10	NULL	0	NULL	statement 3	NULL		occurs because of	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_38	12738681	23 The authors suggested that apoA-I is likely bound to phosphatidylserine (PS) that is presented to the exofacial leaflet by the "`floppase"` activity of ABCA1 because PS levels on the exofacial leaflet are increased by ABCA1 expression.	bind
27145	1	7365	5	13	NULL	NULL	NULL	CRP	GP		bind					LDL	GP	oxidized			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_126	15692104	23 We found that DLH3, but not 4E6 and polyclonal antibodies to apoB, effectively competes with CRP and annexin binding to oxidized LDL, suggesting that both ligands bind to the choline head group of oxidized phospholipids present in the LDL and that specific sequences of the apoB were not essential.	bind
27146	2	7365	5	13	NULL	NULL	NULL	annexin	GP		bind					LDL	GP	oxidized			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_126	15692104	23 We found that DLH3, but not 4E6 and polyclonal antibodies to apoB, effectively competes with CRP and annexin binding to oxidized LDL, suggesting that both ligands bind to the choline head group of oxidized phospholipids present in the LDL and that specific sequences of the apoB were not essential.	bind
27147	4	7365	5	13	NULL	NULL	NULL	statement 3	Process		competes with		effectively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_126	15692104	23 We found that DLH3, but not 4E6 and polyclonal antibodies to apoB, effectively competes with CRP and annexin binding to oxidized LDL, suggesting that both ligands bind to the choline head group of oxidized phospholipids present in the LDL and that specific sequences of the apoB were not essential.	bind
27148	5	7365	5	13	NULL	NULL	NULL	statement 3	Process		competes with		effectively			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_126	15692104	23 We found that DLH3, but not 4E6 and polyclonal antibodies to apoB, effectively competes with CRP and annexin binding to oxidized LDL, suggesting that both ligands bind to the choline head group of oxidized phospholipids present in the LDL and that specific sequences of the apoB were not essential.	bind
27149	6	7365	5	13	NULL	NULL	NULL	4E6	GP		does not compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_126	15692104	23 We found that DLH3, but not 4E6 and polyclonal antibodies to apoB, effectively competes with CRP and annexin binding to oxidized LDL, suggesting that both ligands bind to the choline head group of oxidized phospholipids present in the LDL and that specific sequences of the apoB were not essential.	bind
27150	7	7365	5	13	NULL	NULL	NULL	4E6	GP		does not compete with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_126	15692104	23 We found that DLH3, but not 4E6 and polyclonal antibodies to apoB, effectively competes with CRP and annexin binding to oxidized LDL, suggesting that both ligands bind to the choline head group of oxidized phospholipids present in the LDL and that specific sequences of the apoB were not essential.	bind
27151	8	7365	5	13	NULL	NULL	NULL	polyclonal antibodies to apoB	GP		does not compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_126	15692104	23 We found that DLH3, but not 4E6 and polyclonal antibodies to apoB, effectively competes with CRP and annexin binding to oxidized LDL, suggesting that both ligands bind to the choline head group of oxidized phospholipids present in the LDL and that specific sequences of the apoB were not essential.	bind
27152	9	7365	5	13	NULL	NULL	NULL	polyclonal antibodies to apoB	GP		does not compete with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_126	15692104	23 We found that DLH3, but not 4E6 and polyclonal antibodies to apoB, effectively competes with CRP and annexin binding to oxidized LDL, suggesting that both ligands bind to the choline head group of oxidized phospholipids present in the LDL and that specific sequences of the apoB were not essential.	bind
27153	10	7365	5	13	NULL	NULL	NULL	oxidized phospholipids	Chemical	choline head group of	is present in					LDL	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_126	15692104	23 We found that DLH3, but not 4E6 and polyclonal antibodies to apoB, effectively competes with CRP and annexin binding to oxidized LDL, suggesting that both ligands bind to the choline head group of oxidized phospholipids present in the LDL and that specific sequences of the apoB were not essential.	bind
27155	11	7365	5	13	NULL	NULL	NULL	CRP	GP		bind					statement 10	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_126	15692104	23 We found that DLH3, but not 4E6 and polyclonal antibodies to apoB, effectively competes with CRP and annexin binding to oxidized LDL, suggesting that both ligands bind to the choline head group of oxidized phospholipids present in the LDL and that specific sequences of the apoB were not essential.	bind
27157	12	7365	5	13	NULL	NULL	NULL	annexin	GP		bind					statement 10	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_126	15692104	23 We found that DLH3, but not 4E6 and polyclonal antibodies to apoB, effectively competes with CRP and annexin binding to oxidized LDL, suggesting that both ligands bind to the choline head group of oxidized phospholipids present in the LDL and that specific sequences of the apoB were not essential.	bind
27159	13	7365	5	13	NULL	NULL	NULL	apoB	GP	specific sequences of	is not essential for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_126	15692104	23 We found that DLH3, but not 4E6 and polyclonal antibodies to apoB, effectively competes with CRP and annexin binding to oxidized LDL, suggesting that both ligands bind to the choline head group of oxidized phospholipids present in the LDL and that specific sequences of the apoB were not essential.	bind
27160	14	7365	5	13	NULL	NULL	NULL	apoB	GP	specific sequences of	is not essential for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_126	15692104	23 We found that DLH3, but not 4E6 and polyclonal antibodies to apoB, effectively competes with CRP and annexin binding to oxidized LDL, suggesting that both ligands bind to the choline head group of oxidized phospholipids present in the LDL and that specific sequences of the apoB were not essential.	bind
27161	3	7365	5	13	NULL	NULL	NULL	DLH3	GP		bind					LDL	GP	oxidized			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_126	15692104	23 We found that DLH3, but not 4E6 and polyclonal antibodies to apoB, effectively competes with CRP and annexin binding to oxidized LDL, suggesting that both ligands bind to the choline head group of oxidized phospholipids present in the LDL and that specific sequences of the apoB were not essential.	bind
29410	1	7365	7	NULL	NULL	0	NULL	 CRP	NULL		bind	NULL				LDL	NULL	oxidized	choline head group 		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_126	15692104	23 We found that DLH3, but not 4E6 and polyclonal antibodies to apoB, effectively competes with CRP and annexin binding to oxidized LDL, suggesting that both ligands bind to the choline head group of oxidized phospholipids present in the LDL and that specific sequences of the apoB were not essential.	bind
29411	2	7365	7	NULL	NULL	0	NULL	annexin 	NULL		bind	NULL				LDL	NULL	oxidized	choline head group 		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_126	15692104	23 We found that DLH3, but not 4E6 and polyclonal antibodies to apoB, effectively competes with CRP and annexin binding to oxidized LDL, suggesting that both ligands bind to the choline head group of oxidized phospholipids present in the LDL and that specific sequences of the apoB were not essential.	bind
29412	3	7365	7	NULL	NULL	0	NULL	DLH3	NULL		bind	NULL				LDL	NULL	oxidized			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_126	15692104	23 We found that DLH3, but not 4E6 and polyclonal antibodies to apoB, effectively competes with CRP and annexin binding to oxidized LDL, suggesting that both ligands bind to the choline head group of oxidized phospholipids present in the LDL and that specific sequences of the apoB were not essential.	bind
29413	4	7365	7	NULL	NULL	0	NULL	statement 3	NULL		compete with	NULL	effectively			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_126	15692104	23 We found that DLH3, but not 4E6 and polyclonal antibodies to apoB, effectively competes with CRP and annexin binding to oxidized LDL, suggesting that both ligands bind to the choline head group of oxidized phospholipids present in the LDL and that specific sequences of the apoB were not essential.	bind
29414	5	7365	7	NULL	NULL	0	NULL	statement 3	NULL		compete with	NULL	effectively			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_126	15692104	23 We found that DLH3, but not 4E6 and polyclonal antibodies to apoB, effectively competes with CRP and annexin binding to oxidized LDL, suggesting that both ligands bind to the choline head group of oxidized phospholipids present in the LDL and that specific sequences of the apoB were not essential.	bind
29415	6	7365	7	NULL	NULL	0	NULL	4E6	NULL		does not compete with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_126	15692104	23 We found that DLH3, but not 4E6 and polyclonal antibodies to apoB, effectively competes with CRP and annexin binding to oxidized LDL, suggesting that both ligands bind to the choline head group of oxidized phospholipids present in the LDL and that specific sequences of the apoB were not essential.	bind
29416	7	7365	7	NULL	NULL	0	NULL	4E6	NULL		does not compete with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_126	15692104	23 We found that DLH3, but not 4E6 and polyclonal antibodies to apoB, effectively competes with CRP and annexin binding to oxidized LDL, suggesting that both ligands bind to the choline head group of oxidized phospholipids present in the LDL and that specific sequences of the apoB were not essential.	bind
29417	8	7365	7	NULL	NULL	0	NULL	polyclonal antibodies apoB	NULL		does not compete with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_126	15692104	23 We found that DLH3, but not 4E6 and polyclonal antibodies to apoB, effectively competes with CRP and annexin binding to oxidized LDL, suggesting that both ligands bind to the choline head group of oxidized phospholipids present in the LDL and that specific sequences of the apoB were not essential.	bind
29418	9	7365	7	NULL	NULL	0	NULL	polyclonal antibodies apoB	NULL		does not compete with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_126	15692104	23 We found that DLH3, but not 4E6 and polyclonal antibodies to apoB, effectively competes with CRP and annexin binding to oxidized LDL, suggesting that both ligands bind to the choline head group of oxidized phospholipids present in the LDL and that specific sequences of the apoB were not essential.	bind
29419	10	7365	7	NULL	NULL	0	NULL	apoB	NULL	specific sequences of 	is not required for	NULL				LDL	NULL	binding to			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_126	15692104	23 We found that DLH3, but not 4E6 and polyclonal antibodies to apoB, effectively competes with CRP and annexin binding to oxidized LDL, suggesting that both ligands bind to the choline head group of oxidized phospholipids present in the LDL and that specific sequences of the apoB were not essential.	bind
27172	1	7366	5	13	NULL	NULL	NULL	CREB	GP	phosphorylated	bind						NucleicAcid			CRE sites	NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_17_2088_s_174	11673351	23, 24, 34 A functional relevance for CREB-dependent transcription in the heart derives from studies in human failing and nonfailing heart samples, where binding of phosphorylated CREB to CRE sites has been demonstrated.	bind
29420	1	7366	7	NULL	NULL	0	NULL	CREB	NULL	phosphorylated	binds to	NULL					NULL			CRE sites	NULL		0	NULL	NULL	NULL	gw60_circulation_104_17_2088_s_174	11673351	23, 24, 34 A functional relevance for CREB-dependent transcription in the heart derives from studies in human failing and nonfailing heart samples, where binding of phosphorylated CREB to CRE sites has been demonstrated.	bind
27173	1	7367	5	13	NULL	NULL	NULL	CREB	GP		bind					Rac1 gene	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1634_s_163	15242860	23,24  Our data also indicated that CREB phosphorylation did not increase CREB binding to Rac1 gene promoter.	bind
27174	2	7367	5	13	NULL	NULL	NULL	CREB	GP	phosphorylation	does not increase					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1634_s_163	15242860	23,24  Our data also indicated that CREB phosphorylation did not increase CREB binding to Rac1 gene promoter.	bind
29421	1	7367	7	NULL	NULL	0	NULL	CREB 	NULL		bind	NULL				Rac1 gene	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1634_s_163	15242860	23,24  Our data also indicated that CREB phosphorylation did not increase CREB binding to Rac1 gene promoter.	bind
29422	2	7367	7	NULL	NULL	0	NULL	CREB	NULL	phosphorylation of	does not increase	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1634_s_163	15242860	23,24  Our data also indicated that CREB phosphorylation did not increase CREB binding to Rac1 gene promoter.	bind
27175	1	7368	5	13	NULL	NULL	NULL	EphB4	GP		bind		specifically			ephrin-B2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_17_2210_s_225	15851594	23,24  Whereas EphB4 showed specific binding to ephrin-B2 with its essential role for vascular development, 22,24  EphB3 and EphB2 show less specific binding to ephrin-B2 without their critical role for vascular development.	bind
27176	2	7368	5	13	NULL	NULL	NULL	EphB4	GP		plays a role in		essential			vascular development	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_17_2210_s_225	15851594	23,24  Whereas EphB4 showed specific binding to ephrin-B2 with its essential role for vascular development, 22,24  EphB3 and EphB2 show less specific binding to ephrin-B2 without their critical role for vascular development.	bind
27177	3	7368	5	13	NULL	NULL	NULL	EphB3	GP		bind		less specific			ephrin-B2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_17_2210_s_225	15851594	23,24  Whereas EphB4 showed specific binding to ephrin-B2 with its essential role for vascular development, 22,24  EphB3 and EphB2 show less specific binding to ephrin-B2 without their critical role for vascular development.	bind
27178	4	7368	5	13	NULL	NULL	NULL	EphB3	GP		does not play a role in		critical			vascular development	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_17_2210_s_225	15851594	23,24  Whereas EphB4 showed specific binding to ephrin-B2 with its essential role for vascular development, 22,24  EphB3 and EphB2 show less specific binding to ephrin-B2 without their critical role for vascular development.	bind
27179	5	7368	5	13	NULL	NULL	NULL	EphB2	GP		bind		less specific			ephrin-B2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_17_2210_s_225	15851594	23,24  Whereas EphB4 showed specific binding to ephrin-B2 with its essential role for vascular development, 22,24  EphB3 and EphB2 show less specific binding to ephrin-B2 without their critical role for vascular development.	bind
27180	6	7368	5	13	NULL	NULL	NULL	EphB2	GP		does not play a role in		critical			vascular development	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_17_2210_s_225	15851594	23,24  Whereas EphB4 showed specific binding to ephrin-B2 with its essential role for vascular development, 22,24  EphB3 and EphB2 show less specific binding to ephrin-B2 without their critical role for vascular development.	bind
29423	1	7368	7	NULL	NULL	0	NULL	EphB4	NULL		binds	NULL	specifically			ephrin-B2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_111_17_2210_s_225	15851594	23,24  Whereas EphB4 showed specific binding to ephrin-B2 with its essential role for vascular development, 22,24  EphB3 and EphB2 show less specific binding to ephrin-B2 without their critical role for vascular development.	bind
29424	2	7368	7	10	NULL	0	NULL	statement 1			plays a role in		essential			vascular development					NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_17_2210_s_225	15851594	23,24  Whereas EphB4 showed specific binding to ephrin-B2 with its essential role for vascular development, 22,24  EphB3 and EphB2 show less specific binding to ephrin-B2 without their critical role for vascular development.	bind
29425	3	7368	7	NULL	NULL	0	NULL	EphB3	NULL		binds	NULL	less specific			 ephrin-B2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_111_17_2210_s_225	15851594	23,24  Whereas EphB4 showed specific binding to ephrin-B2 with its essential role for vascular development, 22,24  EphB3 and EphB2 show less specific binding to ephrin-B2 without their critical role for vascular development.	bind
29426	4	7368	7	NULL	NULL	0	NULL	 EphB2	NULL		bind	NULL	less specific			ephrin-B2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_111_17_2210_s_225	15851594	23,24  Whereas EphB4 showed specific binding to ephrin-B2 with its essential role for vascular development, 22,24  EphB3 and EphB2 show less specific binding to ephrin-B2 without their critical role for vascular development.	bind
29427	5	7368	7	NULL	NULL	0	NULL	statement 3	NULL		does not play a role in	NULL				vascular development	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_111_17_2210_s_225	15851594	23,24  Whereas EphB4 showed specific binding to ephrin-B2 with its essential role for vascular development, 22,24  EphB3 and EphB2 show less specific binding to ephrin-B2 without their critical role for vascular development.	bind
29428	6	7368	7	NULL	NULL	0	NULL	statement 4	NULL		does not play a role in	NULL				vascular development	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_111_17_2210_s_225	15851594	23,24  Whereas EphB4 showed specific binding to ephrin-B2 with its essential role for vascular development, 22,24  EphB3 and EphB2 show less specific binding to ephrin-B2 without their critical role for vascular development.	bind
27195	1	7369	5	13	NULL	NULL	NULL	apoA-I	GP		bind								W590S		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_55	12738681	23,32  The moderate increase in apoA-I binding to W590S may imply that dissociation of apoA-I from ABCA1 could be facilitated by lipid efflux to apolipoproteins bound to ABCA1 and is consistent with the earlier finding that ABCA1 binds apoA-I but not HDL3.	bind
27196	2	7369	5	13	NULL	NULL	NULL	apoA-I	GP		dissociates from					ABCA1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_55	12738681	23,32  The moderate increase in apoA-I binding to W590S may imply that dissociation of apoA-I from ABCA1 could be facilitated by lipid efflux to apolipoproteins bound to ABCA1 and is consistent with the earlier finding that ABCA1 binds apoA-I but not HDL3.	bind
27197	3	7369	5	13	NULL	NULL	NULL	apolipoproteins	GP		bind					ABCA1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_55	12738681	23,32  The moderate increase in apoA-I binding to W590S may imply that dissociation of apoA-I from ABCA1 could be facilitated by lipid efflux to apolipoproteins bound to ABCA1 and is consistent with the earlier finding that ABCA1 binds apoA-I but not HDL3.	bind
27198	4	7369	5	13	NULL	NULL	NULL	statement 2	Process		is facilitated by					statement 3	Process	lipid efflux to			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_55	12738681	23,32  The moderate increase in apoA-I binding to W590S may imply that dissociation of apoA-I from ABCA1 could be facilitated by lipid efflux to apolipoproteins bound to ABCA1 and is consistent with the earlier finding that ABCA1 binds apoA-I but not HDL3.	bind
27199	5	7369	5	13	NULL	NULL	NULL	statement 1	Process	moderate increase in	imply		may			statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_55	12738681	23,32  The moderate increase in apoA-I binding to W590S may imply that dissociation of apoA-I from ABCA1 could be facilitated by lipid efflux to apolipoproteins bound to ABCA1 and is consistent with the earlier finding that ABCA1 binds apoA-I but not HDL3.	bind
27200	6	7369	5	13	NULL	NULL	NULL	ABCA1	GP		bind					apoA-I	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_55	12738681	23,32  The moderate increase in apoA-I binding to W590S may imply that dissociation of apoA-I from ABCA1 could be facilitated by lipid efflux to apolipoproteins bound to ABCA1 and is consistent with the earlier finding that ABCA1 binds apoA-I but not HDL3.	bind
27201	7	7369	5	13	NULL	NULL	NULL	ABCA1	GP		does not bind					HDL3	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_55	12738681	23,32  The moderate increase in apoA-I binding to W590S may imply that dissociation of apoA-I from ABCA1 could be facilitated by lipid efflux to apolipoproteins bound to ABCA1 and is consistent with the earlier finding that ABCA1 binds apoA-I but not HDL3.	bind
29429	1	7369	7	NULL	NULL	0	NULL	apoA-I	NULL		binds to	NULL					NULL		W590S 		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_55	12738681	23,32  The moderate increase in apoA-I binding to W590S may imply that dissociation of apoA-I from ABCA1 could be facilitated by lipid efflux to apolipoproteins bound to ABCA1 and is consistent with the earlier finding that ABCA1 binds apoA-I but not HDL3.	bind
29430	2	7369	7	NULL	NULL	0	NULL	apoA-I	NULL		dissociates from	NULL				ABCA1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_55	12738681	23,32  The moderate increase in apoA-I binding to W590S may imply that dissociation of apoA-I from ABCA1 could be facilitated by lipid efflux to apolipoproteins bound to ABCA1 and is consistent with the earlier finding that ABCA1 binds apoA-I but not HDL3.	bind
29431	3	7369	7	NULL	NULL	0	NULL	statement 1	NULL	increase in	imply	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_55	12738681	23,32  The moderate increase in apoA-I binding to W590S may imply that dissociation of apoA-I from ABCA1 could be facilitated by lipid efflux to apolipoproteins bound to ABCA1 and is consistent with the earlier finding that ABCA1 binds apoA-I but not HDL3.	bind
29432	4	7369	7	NULL	NULL	0	NULL	apolipoproteins	NULL		bind	NULL				ABCA1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_55	12738681	23,32  The moderate increase in apoA-I binding to W590S may imply that dissociation of apoA-I from ABCA1 could be facilitated by lipid efflux to apolipoproteins bound to ABCA1 and is consistent with the earlier finding that ABCA1 binds apoA-I but not HDL3.	bind
29433	5	7369	7	NULL	NULL	0	NULL	statement 4	NULL	lipid efflux to	facilitate	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_55	12738681	23,32  The moderate increase in apoA-I binding to W590S may imply that dissociation of apoA-I from ABCA1 could be facilitated by lipid efflux to apolipoproteins bound to ABCA1 and is consistent with the earlier finding that ABCA1 binds apoA-I but not HDL3.	bind
29434	6	7369	7	NULL	NULL	0	NULL	ABCA1	NULL		binds	NULL				apoA-I	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_55	12738681	23,32  The moderate increase in apoA-I binding to W590S may imply that dissociation of apoA-I from ABCA1 could be facilitated by lipid efflux to apolipoproteins bound to ABCA1 and is consistent with the earlier finding that ABCA1 binds apoA-I but not HDL3.	bind
29435	7	7369	7	NULL	NULL	0	NULL	ABCA1	NULL		does not bind	NULL				HDL3	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_55	12738681	23,32  The moderate increase in apoA-I binding to W590S may imply that dissociation of apoA-I from ABCA1 could be facilitated by lipid efflux to apolipoproteins bound to ABCA1 and is consistent with the earlier finding that ABCA1 binds apoA-I but not HDL3.	bind
27202	1	7370	5	13	NULL	NULL	NULL	VN	GP	surface-bound serum-derived	bind					uPAR	GP				NULL	 cells cultured in serum-containing medium	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2251_s_155	15458976	23,38  When cultured in serum-containing medium, cells may have surface-bound serum-derived VN that binds uPAR and Mac-1, thereby influencing cell adhesion.	bind
27203	2	7370	5	13	NULL	NULL	NULL	statement 1	Process		influence					cell adhesion	Process				NULL	cells cultured in serum-containing medium	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2251_s_155	15458976	23,38  When cultured in serum-containing medium, cells may have surface-bound serum-derived VN that binds uPAR and Mac-1, thereby influencing cell adhesion.	bind
27204	3	7370	5	13	NULL	NULL	NULL	VN	GP	surface-bound serum-derived	bind					Mac-1	GP				NULL	cells cultured in serum-containing medium	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2251_s_155	15458976	23,38  When cultured in serum-containing medium, cells may have surface-bound serum-derived VN that binds uPAR and Mac-1, thereby influencing cell adhesion.	bind
27205	4	7370	5	13	NULL	NULL	NULL	statement 2	Process		influence					cell adhesion	Process				NULL	cells cultured in serum-containing medium	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2251_s_155	15458976	23,38  When cultured in serum-containing medium, cells may have surface-bound serum-derived VN that binds uPAR and Mac-1, thereby influencing cell adhesion.	bind
29436	1	7370	7	NULL	NULL	0	NULL	VN	NULL	surface-bound serum-derived	binds	NULL				uPAR	NULL				NULL	serum-containing medium	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2251_s_155	15458976	23,38  When cultured in serum-containing medium, cells may have surface-bound serum-derived VN that binds uPAR and Mac-1, thereby influencing cell adhesion.	bind
29437	2	7370	7	NULL	NULL	0	NULL	VN	NULL	surface-bound serum-derived	binds	NULL				Mac-1	NULL				NULL	serum-containing medium	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2251_s_155	15458976	23,38  When cultured in serum-containing medium, cells may have surface-bound serum-derived VN that binds uPAR and Mac-1, thereby influencing cell adhesion.	bind
29438	3	7370	7	10	NULL	0	NULL	statement 1			influence					cell adhesion					NULL	serum-containing medium	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2251_s_155	15458976	23,38  When cultured in serum-containing medium, cells may have surface-bound serum-derived VN that binds uPAR and Mac-1, thereby influencing cell adhesion.	bind
29439	4	7370	7	10	NULL	0	NULL	statement 2			influence					cell adhesion					NULL	serum-containing medium	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2251_s_155	15458976	23,38  When cultured in serum-containing medium, cells may have surface-bound serum-derived VN that binds uPAR and Mac-1, thereby influencing cell adhesion.	bind
27206	1	7372	5	13	NULL	NULL	NULL	dystrophin	GP		bind			N-terminus		actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_9_1256_s_143	11238270	24  At the N-terminus, dystrophin binds to actin.	bind
29440	1	7372	7	NULL	NULL	0	NULL	dystrophin	NULL		binds to	NULL		N-terminus		actin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_9_1256_s_143	11238270	24  At the N-terminus, dystrophin binds to actin.	bind
27207	1	7373	5	13	NULL	NULL	NULL	p27	GP		bind			69-amino-acid amino-terminal inhibitory domain		cyclin A-CDK2	GP	phosphorylated			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_2_313_s_36	10027389	24  Examination of the crystal structure of the 69-amino-acid amino-terminal inhibitory domain of p27 bound to the phosphorylated cyclin A-CDK2 showed that p27 binding causes large conformational changes in and around the catalytic cleft of CDK2 24  and that p27 has separate binding sites on the cyclin and CDK subunits.	bind
27208	2	7373	5	13	NULL	NULL	NULL	statement 1	Process		results in					CDK2	GP	large conformational changes in and around	catalytic cleft		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_2_313_s_36	10027389	24  Examination of the crystal structure of the 69-amino-acid amino-terminal inhibitory domain of p27 bound to the phosphorylated cyclin A-CDK2 showed that p27 binding causes large conformational changes in and around the catalytic cleft of CDK2 24  and that p27 has separate binding sites on the cyclin and CDK subunits.	bind
27209	3	7373	5	13	NULL	NULL	NULL	p27	GP		contains					cyclin	GP		binding site		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_2_313_s_36	10027389	24  Examination of the crystal structure of the 69-amino-acid amino-terminal inhibitory domain of p27 bound to the phosphorylated cyclin A-CDK2 showed that p27 binding causes large conformational changes in and around the catalytic cleft of CDK2 24  and that p27 has separate binding sites on the cyclin and CDK subunits.	bind
27210	4	7373	5	13	NULL	NULL	NULL	p27	GP		contains					CDK subunits	GP		binding site		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_2_313_s_36	10027389	24  Examination of the crystal structure of the 69-amino-acid amino-terminal inhibitory domain of p27 bound to the phosphorylated cyclin A-CDK2 showed that p27 binding causes large conformational changes in and around the catalytic cleft of CDK2 24  and that p27 has separate binding sites on the cyclin and CDK subunits.	bind
29441	1	7373	7	NULL	NULL	0	NULL	p27	NULL		bind	NULL		69-amino-acid amino-terminal inhibitory domain 		cyclin A-CDK2 	NULL	phosphorylated			NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_2_313_s_36	10027389	24  Examination of the crystal structure of the 69-amino-acid amino-terminal inhibitory domain of p27 bound to the phosphorylated cyclin A-CDK2 showed that p27 binding causes large conformational changes in and around the catalytic cleft of CDK2 24  and that p27 has separate binding sites on the cyclin and CDK subunits.	bind
29442	2	7373	7	NULL	NULL	0	NULL	statement 1	NULL		cause	NULL				CDK2	NULL	conformational changes in and around	catalytic cleft		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_2_313_s_36	10027389	24  Examination of the crystal structure of the 69-amino-acid amino-terminal inhibitory domain of p27 bound to the phosphorylated cyclin A-CDK2 showed that p27 binding causes large conformational changes in and around the catalytic cleft of CDK2 24  and that p27 has separate binding sites on the cyclin and CDK subunits.	bind
29443	3	7373	7	NULL	NULL	0	NULL	cyclin	NULL		contains	NULL				p27	NULL		binding site		NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_2_313_s_36	10027389	24  Examination of the crystal structure of the 69-amino-acid amino-terminal inhibitory domain of p27 bound to the phosphorylated cyclin A-CDK2 showed that p27 binding causes large conformational changes in and around the catalytic cleft of CDK2 24  and that p27 has separate binding sites on the cyclin and CDK subunits.	bind
29444	4	7373	7	NULL	NULL	0	NULL	CDK subunits	NULL		contains	NULL				p27	NULL		binding site		NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_2_313_s_36	10027389	24  Examination of the crystal structure of the 69-amino-acid amino-terminal inhibitory domain of p27 bound to the phosphorylated cyclin A-CDK2 showed that p27 binding causes large conformational changes in and around the catalytic cleft of CDK2 24  and that p27 has separate binding sites on the cyclin and CDK subunits.	bind
27211	1	7374	5	13	NULL	NULL	NULL	FK506	Chemical		bind					FKBP	GP				NULL	in cardiomyocytes	NULL	NULL	NULL	NULL	gw60_circulation_100_24_2449_s_149	10595959	24  In cardiomyocytes, it has been reported that FK506 binds to FKBP and opens the ryanodine receptor, resulting in an increase in intracellular calcium concentration.	bind
27212	2	7374	5	13	NULL	NULL	NULL	statement 1	Process		opens					ryanodine receptor	GP				NULL	cardiomyocytes	NULL	NULL	NULL	NULL	gw60_circulation_100_24_2449_s_149	10595959	24  In cardiomyocytes, it has been reported that FK506 binds to FKBP and opens the ryanodine receptor, resulting in an increase in intracellular calcium concentration.	bind
27213	3	7374	5	13	NULL	NULL	NULL	statement 2	Process		results in					calcium concentration	Chemical	increase in intracellular			NULL	cardiomyocytes	NULL	NULL	NULL	NULL	gw60_circulation_100_24_2449_s_149	10595959	24  In cardiomyocytes, it has been reported that FK506 binds to FKBP and opens the ryanodine receptor, resulting in an increase in intracellular calcium concentration.	bind
29445	1	7374	7	NULL	NULL	0	NULL	FK506	NULL		binds to	NULL				FKBP	NULL				NULL	cardiomyocytes	NULL	NULL	NULL	NULL	gw60_circulation_100_24_2449_s_149	10595959	24  In cardiomyocytes, it has been reported that FK506 binds to FKBP and opens the ryanodine receptor, resulting in an increase in intracellular calcium concentration.	bind
29446	2	7374	7	NULL	NULL	0	NULL	statement 1	NULL		opens	NULL				ryanodine receptor	NULL				NULL	cardiomyocytes	0	NULL	NULL	NULL	gw60_circulation_100_24_2449_s_149	10595959	24  In cardiomyocytes, it has been reported that FK506 binds to FKBP and opens the ryanodine receptor, resulting in an increase in intracellular calcium concentration.	bind
29447	3	7374	7	NULL	NULL	0	NULL	statement 2	NULL		increase	NULL				calcium	NULL	intracellular concentration of			NULL	cardiomyocytes	NULL	NULL	NULL	NULL	gw60_circulation_100_24_2449_s_149	10595959	24  In cardiomyocytes, it has been reported that FK506 binds to FKBP and opens the ryanodine receptor, resulting in an increase in intracellular calcium concentration.	bind
27214	1	7375	5	13	NULL	NULL	NULL	LDL particles	GP		bind					mast cell granule remnants	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_11_2047_s_144	7583588	24  Moreover, a specific mechanism that increases the strength of binding between LDL particles and mast cell granule remnants was recently discovered.	bind
29448	1	7375	7	NULL	NULL	0	NULL	 LDL particles	NULL		bind	NULL				 mast cell granule remnants	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_11_2047_s_144	7583588	24  Moreover, a specific mechanism that increases the strength of binding between LDL particles and mast cell granule remnants was recently discovered.	bind
27215	1	7376	5	13	NULL	NULL	NULL	IgG	GP		bind					MDA-LDL antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_18_2277_s_43	11342477	24  The amount of IgG bound to the MDA-LDL antigen was detected with alkaline phosphatase - labeled anti-mouse IgG.	bind
29449	1	7376	7	NULL	NULL	0	NULL	IgG	NULL		bind	NULL				MDA-LDL antigen	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_18_2277_s_43	11342477	24  The amount of IgG bound to the MDA-LDL antigen was detected with alkaline phosphatase - labeled anti-mouse IgG.	bind
27216	1	7377	5	13	NULL	NULL	NULL	IL-1R1	GP		is					IL-1 receptor 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
27217	2	7377	5	13	NULL	NULL	NULL	 IL-1	GP		bind					IL-1R1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
27218	3	7377	5	13	NULL	NULL	NULL	IL-1	GP		bind					accessory protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
27219	4	7377	5	13	NULL	NULL	NULL	statement 2	Process		triggers					signal transduction	Process	intracellular			NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
27220	5	7377	5	13	NULL	NULL	NULL	statement 3	Process		triggers					signal transduction	Process	intracellular			NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
27221	6	7377	5	13	NULL	NULL	NULL	statement 4 & 5	Process		activates					vasoactive substances	GP	synthesis of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
27222	7	7377	5	13	NULL	NULL	NULL	statement 4 & 5	Process		activates					growth factors	GP	synthesis of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
27223	8	7377	5	13	NULL	NULL	NULL	statement 4 & 5	Process		activates					cytokines	GP	synthesis of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
27224	9	7377	5	13	NULL	NULL	NULL	chemokines	GP		attract					monocyte-derived cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
27225	10	7377	5	13	NULL	NULL	NULL	statement 2	Process		increases					adhesion molecules	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
27226	11	7377	5	13	NULL	NULL	NULL	statement 3	Process		increases					adhesion molecules	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
27227	12	7377	5	13	NULL	NULL	NULL	statement 2	Process		increases					statement 9	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
27228	13	7377	5	13	NULL	NULL	NULL	statement 3	Process		increases					statement 9	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
27229	14	7377	5	13	NULL	NULL	NULL	statement 2	Process		enhances					diapedesis	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
27230	15	7377	5	13	NULL	NULL	NULL	statement 3	Process		enhances					diapedesis	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
29450	1	7377	7	NULL	NULL	0	NULL	 IL-1	NULL		bind	NULL				IL-1R1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
29451	2	7377	7	NULL	NULL	0	NULL	IL-1	NULL		binds	NULL				IL-1R1 accessory protein	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
29452	3	7377	7	NULL	NULL	0	NULL	statement 1	NULL		triggers	NULL				signal transduction	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
29453	4	7377	7	NULL	NULL	0	NULL	statement 2	NULL		triggers	NULL				signal transduction	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
29454	5	7377	7	NULL	NULL	0	NULL	statement 3	NULL		activates	NULL				vasoactive substances	NULL	synthesis of			NULL		0	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
29455	6	7377	7	NULL	NULL	0	NULL	statement 4	NULL		activates	NULL				vasoactive substances	NULL	synthesis of			NULL		0	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
29456	7	7377	7	NULL	NULL	0	NULL	statement 3	NULL		activates	NULL				growth factors	NULL	synthesis of			NULL		0	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
29457	8	7377	7	NULL	NULL	0	NULL	statement 4	NULL		activates	NULL				growth factors	NULL	synthesis of			NULL		0	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
29458	9	7377	7	NULL	NULL	0	NULL	statement 3	NULL		activates	NULL				cytokines	NULL	synthesis of			NULL		0	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
29459	10	7377	7	NULL	NULL	0	NULL	statement 4	NULL		activates	NULL				cytokines	NULL	synthesis of			NULL		0	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
29460	11	7377	7	NULL	NULL	0	NULL	statement 3	NULL		increase	NULL				vascular adhesion molecules	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
29461	12	7377	7	NULL	NULL	0	NULL	statement 4	NULL		increase	NULL				vascular adhesion molecules	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
29464	13	7377	7	NULL	NULL	0	NULL	statement 3	NULL		increase	NULL				chemokines	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
29465	14	7377	7	NULL	NULL	0	NULL	statement 4	NULL		increase	NULL				chemokines	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
29466	15	7377	7	NULL	NULL	0	NULL	chemokines	NULL		attract	NULL				monocyte-derived cells	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
29467	16	7377	7	NULL	NULL	0	NULL	statement 15	NULL		enhance	NULL				diapedesis	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
29468	17	7377	7	NULL	NULL	0	NULL	chemokines	NULL		stimulate	NULL				monocyte-derived cells	NULL	proliferation of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
29469	18	7377	7	NULL	NULL	0	NULL	chemokines	NULL		stimulate	NULL				monocyte-derived cells	NULL	differentiation of			NULL		0	NULL	NULL	NULL	gw70_circulation_110_12_1678_s_31	15353494	24 - 26   IL-1 binding to the IL-1 receptor 1 (IL-1R1) and its accessory protein triggers intracellular signal transduction to activate the synthesis of vasoactive substances, growth factors, and cytokines, as well as increases the expression of vascular adhesion molecules and chemokines that attract monocyte-derived cells, enhance diapedesis, and stimulate their proliferation and differentiation.	bind
27231	1	7378	5	13	NULL	NULL	NULL	TNF-alpha 	GP		combines with					IFN-gamma	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_2_227_s_136	11156857	24 25 26  For example, the combination of TNF-alpha and IFN-gamma activates the human class I MHC promoter synergistically, and this induction requires the binding of both NF-kappaB and IRF-1 to the class I MHC promoter.	bind
27232	2	7378	5	13	NULL	NULL	NULL	NF-kappaB	GP		bind					class I MHC	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_2_227_s_136	11156857	24 25 26  For example, the combination of TNF-alpha and IFN-gamma activates the human class I MHC promoter synergistically, and this induction requires the binding of both NF-kappaB and IRF-1 to the class I MHC promoter.	bind
27233	3	7378	5	13	NULL	NULL	NULL	IRF-1	GP		bind					class I MHC	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_2_227_s_136	11156857	24 25 26  For example, the combination of TNF-alpha and IFN-gamma activates the human class I MHC promoter synergistically, and this induction requires the binding of both NF-kappaB and IRF-1 to the class I MHC promoter.	bind
27234	4	7378	5	13	NULL	NULL	NULL	statement 1	Process		requires					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_2_227_s_136	11156857	24 25 26  For example, the combination of TNF-alpha and IFN-gamma activates the human class I MHC promoter synergistically, and this induction requires the binding of both NF-kappaB and IRF-1 to the class I MHC promoter.	bind
27235	5	7378	5	13	NULL	NULL	NULL	statement 1	Process		requires					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_2_227_s_136	11156857	24 25 26  For example, the combination of TNF-alpha and IFN-gamma activates the human class I MHC promoter synergistically, and this induction requires the binding of both NF-kappaB and IRF-1 to the class I MHC promoter.	bind
46602	6	7378	5	13	NULL	NULL	NULL	statement 1	Process		activates					class I MHC	GP	human		promoter	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_2_227_s_136	11156857	24 25 26  For example, the combination of TNF-alpha and IFN-gamma activates the human class I MHC promoter synergistically, and this induction requires the binding of both NF-kappaB and IRF-1 to the class I MHC promoter.	bind
29471	1	7378	7	NULL	NULL	0	NULL	TNF-alpha	NULL		combines with	NULL				IFN-gamma	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_2_227_s_136	11156857	24 25 26  For example, the combination of TNF-alpha and IFN-gamma activates the human class I MHC promoter synergistically, and this induction requires the binding of both NF-kappaB and IRF-1 to the class I MHC promoter.	bind
29472	2	7378	7	NULL	NULL	0	NULL	statement 1	NULL		activates	NULL				class I MHC	NULL	human		promoter	NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_2_227_s_136	11156857	24 25 26  For example, the combination of TNF-alpha and IFN-gamma activates the human class I MHC promoter synergistically, and this induction requires the binding of both NF-kappaB and IRF-1 to the class I MHC promoter.	bind
29478	3	7378	7	NULL	NULL	0	NULL	statement 2	NULL		occurs synergistically with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_2_227_s_136	11156857	24 25 26  For example, the combination of TNF-alpha and IFN-gamma activates the human class I MHC promoter synergistically, and this induction requires the binding of both NF-kappaB and IRF-1 to the class I MHC promoter.	bind
29479	4	7378	7	NULL	NULL	0	NULL	NF-kappaB 	NULL		binds to	NULL				class I MHC	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_2_227_s_136	11156857	24 25 26  For example, the combination of TNF-alpha and IFN-gamma activates the human class I MHC promoter synergistically, and this induction requires the binding of both NF-kappaB and IRF-1 to the class I MHC promoter.	bind
29480	5	7378	7	NULL	NULL	0	NULL	IRF-1	NULL		binds to	NULL				class I MHC	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_2_227_s_136	11156857	24 25 26  For example, the combination of TNF-alpha and IFN-gamma activates the human class I MHC promoter synergistically, and this induction requires the binding of both NF-kappaB and IRF-1 to the class I MHC promoter.	bind
29481	6	7378	7	NULL	NULL	0	NULL	statement 3	NULL		requires	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_2_227_s_136	11156857	24 25 26  For example, the combination of TNF-alpha and IFN-gamma activates the human class I MHC promoter synergistically, and this induction requires the binding of both NF-kappaB and IRF-1 to the class I MHC promoter.	bind
29482	7	7378	7	NULL	NULL	0	NULL	statement 3	NULL		requires	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_2_227_s_136	11156857	24 25 26  For example, the combination of TNF-alpha and IFN-gamma activates the human class I MHC promoter synergistically, and this induction requires the binding of both NF-kappaB and IRF-1 to the class I MHC promoter.	bind
27236	1	7380	5	13	NULL	NULL	NULL				bind		strongly		palindromic CRE	CREB	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_157	16497991	24 Although palindromic CRE bind strongly to several members of the bZIP family, including CREB, ATF1, ATF2, and c-Jun, variant CRE binds to predominantly ATF2 and c-Jun.	bind
27237	2	7380	5	13	NULL	NULL	NULL				bind		strongly		palindromic CRE	ATF1	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_157	16497991	24 Although palindromic CRE bind strongly to several members of the bZIP family, including CREB, ATF1, ATF2, and c-Jun, variant CRE binds to predominantly ATF2 and c-Jun.	bind
27238	3	7380	5	13	NULL	NULL	NULL				bind		strongly		palindromic CRE	ATF2	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_157	16497991	24 Although palindromic CRE bind strongly to several members of the bZIP family, including CREB, ATF1, ATF2, and c-Jun, variant CRE binds to predominantly ATF2 and c-Jun.	bind
27239	4	7380	5	13	NULL	NULL	NULL				bind		strongly		palindromic CRE	c-Jun	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_157	16497991	24 Although palindromic CRE bind strongly to several members of the bZIP family, including CREB, ATF1, ATF2, and c-Jun, variant CRE binds to predominantly ATF2 and c-Jun.	bind
27240	5	7380	5	13	NULL	NULL	NULL	CREB	GP		is a member of					bZIP family	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_157	16497991	24 Although palindromic CRE bind strongly to several members of the bZIP family, including CREB, ATF1, ATF2, and c-Jun, variant CRE binds to predominantly ATF2 and c-Jun.	bind
27241	6	7380	5	13	NULL	NULL	NULL	ATF1	GP		is a member of					bZIP family	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_157	16497991	24 Although palindromic CRE bind strongly to several members of the bZIP family, including CREB, ATF1, ATF2, and c-Jun, variant CRE binds to predominantly ATF2 and c-Jun.	bind
27242	7	7380	5	13	NULL	NULL	NULL	ATF2	GP		is a member of					bZIP family	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_157	16497991	24 Although palindromic CRE bind strongly to several members of the bZIP family, including CREB, ATF1, ATF2, and c-Jun, variant CRE binds to predominantly ATF2 and c-Jun.	bind
27243	8	7380	5	13	NULL	NULL	NULL	c-Jun	GP		is a member of					bZIP family	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_157	16497991	24 Although palindromic CRE bind strongly to several members of the bZIP family, including CREB, ATF1, ATF2, and c-Jun, variant CRE binds to predominantly ATF2 and c-Jun.	bind
27244	9	7380	5	13	NULL	NULL	NULL			variant	bind		predominantly		CRE	ATF2	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_157	16497991	24 Although palindromic CRE bind strongly to several members of the bZIP family, including CREB, ATF1, ATF2, and c-Jun, variant CRE binds to predominantly ATF2 and c-Jun.	bind
27245	10	7380	5	13	NULL	NULL	NULL			variant	bind		predominantly		CRE	c-Jun	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_157	16497991	24 Although palindromic CRE bind strongly to several members of the bZIP family, including CREB, ATF1, ATF2, and c-Jun, variant CRE binds to predominantly ATF2 and c-Jun.	bind
29483	1	7380	7	NULL	NULL	0	NULL	 	NULL		bind	NULL	strongly		palindromic CRE	CREB	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_157	16497991	24 Although palindromic CRE bind strongly to several members of the bZIP family, including CREB, ATF1, ATF2, and c-Jun, variant CRE binds to predominantly ATF2 and c-Jun.	bind
29484	2	7380	7	NULL	NULL	0	NULL		NULL		bind	NULL	strongly		palindromic CRE	ATF1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_157	16497991	24 Although palindromic CRE bind strongly to several members of the bZIP family, including CREB, ATF1, ATF2, and c-Jun, variant CRE binds to predominantly ATF2 and c-Jun.	bind
29485	3	7380	7	NULL	NULL	0	NULL		NULL		bind	NULL	strongly		palindromic CRE	ATF2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_157	16497991	24 Although palindromic CRE bind strongly to several members of the bZIP family, including CREB, ATF1, ATF2, and c-Jun, variant CRE binds to predominantly ATF2 and c-Jun.	bind
29486	4	7380	7	NULL	NULL	0	NULL		NULL		bind	NULL	strongly		palindromic CRE	c-Jun	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_157	16497991	24 Although palindromic CRE bind strongly to several members of the bZIP family, including CREB, ATF1, ATF2, and c-Jun, variant CRE binds to predominantly ATF2 and c-Jun.	bind
29487	5	7380	7	NULL	NULL	0	NULL		NULL		bind	NULL			variant CRE	ATF2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_157	16497991	24 Although palindromic CRE bind strongly to several members of the bZIP family, including CREB, ATF1, ATF2, and c-Jun, variant CRE binds to predominantly ATF2 and c-Jun.	bind
29488	6	7380	7	NULL	NULL	0	NULL		NULL		bind	NULL			variant CRE	c-Jun	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_157	16497991	24 Although palindromic CRE bind strongly to several members of the bZIP family, including CREB, ATF1, ATF2, and c-Jun, variant CRE binds to predominantly ATF2 and c-Jun.	bind
29489	7	7380	7	NULL	NULL	0	NULL	CREB	NULL		belongs to	NULL				bZIP family	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_157	16497991	24 Although palindromic CRE bind strongly to several members of the bZIP family, including CREB, ATF1, ATF2, and c-Jun, variant CRE binds to predominantly ATF2 and c-Jun.	bind
29490	8	7380	7	NULL	NULL	0	NULL	ATF1	NULL		belongs to	NULL				bZIP family	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_157	16497991	24 Although palindromic CRE bind strongly to several members of the bZIP family, including CREB, ATF1, ATF2, and c-Jun, variant CRE binds to predominantly ATF2 and c-Jun.	bind
29491	9	7380	7	NULL	NULL	0	NULL	ATF2	NULL		belongs to	NULL				bZIP family	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_157	16497991	24 Although palindromic CRE bind strongly to several members of the bZIP family, including CREB, ATF1, ATF2, and c-Jun, variant CRE binds to predominantly ATF2 and c-Jun.	bind
29492	10	7380	7	NULL	NULL	0	NULL	c-Jun	NULL		belongs to	NULL				bZIP family	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_1036_s_157	16497991	24 Although palindromic CRE bind strongly to several members of the bZIP family, including CREB, ATF1, ATF2, and c-Jun, variant CRE binds to predominantly ATF2 and c-Jun.	bind
27246	1	7381	5	13	NULL	NULL	NULL	SRF	GP		bind					SMalpha-actin	GP			CArG containing regions of promoter	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_11_2328_s_190	16151017	24 Although the authors did not find the effect of KLF4 on SRF - DNA binding in EMSA, they observed that overexpression of KLF4 was associated with reduction in SRF binding to CArG containing regions of SMalpha-actin promoter.	bind
27247	2	7381	5	13	NULL	NULL	NULL	KLF4	GP	overexpression of	reduces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_11_2328_s_190	16151017	24 Although the authors did not find the effect of KLF4 on SRF - DNA binding in EMSA, they observed that overexpression of KLF4 was associated with reduction in SRF binding to CArG containing regions of SMalpha-actin promoter.	bind
29493	1	7381	7	NULL	NULL	0	NULL	SRF	NULL		binds	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_11_2328_s_190	16151017	24 Although the authors did not find the effect of KLF4 on SRF - DNA binding in EMSA, they observed that overexpression of KLF4 was associated with reduction in SRF binding to CArG containing regions of SMalpha-actin promoter.	bind
29494	2	7381	7	10	NULL	0	NULL	SRF 	NULL		binds to	NULL				SMalpha-actin	NULL			CArG containing regions of promoter	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_11_2328_s_190	16151017	24 Although the authors did not find the effect of KLF4 on SRF - DNA binding in EMSA, they observed that overexpression of KLF4 was associated with reduction in SRF binding to CArG containing regions of SMalpha-actin promoter.	bind
29495	3	7381	7	NULL	NULL	0	NULL	KLF4	NULL	overexpression	reduce	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_11_2328_s_190	16151017	24 Although the authors did not find the effect of KLF4 on SRF - DNA binding in EMSA, they observed that overexpression of KLF4 was associated with reduction in SRF binding to CArG containing regions of SMalpha-actin promoter.	bind
27248	1	7382	5	13	NULL	NULL	NULL	 iron protoporphyrin IX	Chemical		attached to		covalently			FixL	GP		histidine residue		NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_6_2995_s_29	11248020	24 and  25); ( ii) iron protoporphyrin IX covalently attached to a histidine residue in FixL (sensor protein in  Rhizobium nitrogen fixation pathway; ref.  26); ( iii) flavin adenine dinucleotide noncovalently bound to nitrogen fixation regulatory protein L and  Escherichia coli aerotaxis sensor ( 27-29); and ( iv) FMN noncovalently bound to phototropin ( 9,  12).	bind
27249	2	7382	5	13	NULL	NULL	NULL	FixL	GP		is a type of					sensor protein	GP	Rhizobium nitrogen fixation pathway			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_6_2995_s_29	11248020	24 and  25); ( ii) iron protoporphyrin IX covalently attached to a histidine residue in FixL (sensor protein in  Rhizobium nitrogen fixation pathway; ref.  26); ( iii) flavin adenine dinucleotide noncovalently bound to nitrogen fixation regulatory protein L and  Escherichia coli aerotaxis sensor ( 27-29); and ( iv) FMN noncovalently bound to phototropin ( 9,  12).	bind
27250	3	7382	5	13	NULL	NULL	NULL	flavin adenine dinucleotide	Chemical		bind		noncovalently			nitrogen fixation regulatory protein L	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_6_2995_s_29	11248020	24 and  25); ( ii) iron protoporphyrin IX covalently attached to a histidine residue in FixL (sensor protein in  Rhizobium nitrogen fixation pathway; ref.  26); ( iii) flavin adenine dinucleotide noncovalently bound to nitrogen fixation regulatory protein L and  Escherichia coli aerotaxis sensor ( 27-29); and ( iv) FMN noncovalently bound to phototropin ( 9,  12).	bind
27251	4	7382	5	13	NULL	NULL	NULL	flavin adenine dinucleotide	Chemical		bind		noncovalently			aerotaxis sensor		Escherichia coli			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_6_2995_s_29	11248020	24 and  25); ( ii) iron protoporphyrin IX covalently attached to a histidine residue in FixL (sensor protein in  Rhizobium nitrogen fixation pathway; ref.  26); ( iii) flavin adenine dinucleotide noncovalently bound to nitrogen fixation regulatory protein L and  Escherichia coli aerotaxis sensor ( 27-29); and ( iv) FMN noncovalently bound to phototropin ( 9,  12).	bind
27252	5	7382	5	13	NULL	NULL	NULL	FMN	Chemical		bind		noncovalently			phototropin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_6_2995_s_29	11248020	24 and  25); ( ii) iron protoporphyrin IX covalently attached to a histidine residue in FixL (sensor protein in  Rhizobium nitrogen fixation pathway; ref.  26); ( iii) flavin adenine dinucleotide noncovalently bound to nitrogen fixation regulatory protein L and  Escherichia coli aerotaxis sensor ( 27-29); and ( iv) FMN noncovalently bound to phototropin ( 9,  12).	bind
29496	1	7382	7	NULL	NULL	0	NULL	iron protoporphyrin IX 	NULL		binds	NULL	covalently			FixL	NULL		histidine residue		NULL		0	NULL	NULL	NULL	gw60_pnas_98_6_2995_s_29	11248020	24 and  25); ( ii) iron protoporphyrin IX covalently attached to a histidine residue in FixL (sensor protein in  Rhizobium nitrogen fixation pathway; ref.  26); ( iii) flavin adenine dinucleotide noncovalently bound to nitrogen fixation regulatory protein L and  Escherichia coli aerotaxis sensor ( 27-29); and ( iv) FMN noncovalently bound to phototropin ( 9,  12).	bind
29497	2	7382	7	NULL	NULL	0	NULL	FixL	NULL		is a type of	NULL				sensor protein	NULL	Rhizobium nitrogen fixation pathway			NULL		0	NULL	NULL	NULL	gw60_pnas_98_6_2995_s_29	11248020	24 and  25); ( ii) iron protoporphyrin IX covalently attached to a histidine residue in FixL (sensor protein in  Rhizobium nitrogen fixation pathway; ref.  26); ( iii) flavin adenine dinucleotide noncovalently bound to nitrogen fixation regulatory protein L and  Escherichia coli aerotaxis sensor ( 27-29); and ( iv) FMN noncovalently bound to phototropin ( 9,  12).	bind
29498	3	7382	7	NULL	NULL	0	NULL	flavin adenine dinucleotide 	NULL		bind	NULL	noncovalently			nitrogen fixation regulatory protein L	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_98_6_2995_s_29	11248020	24 and  25); ( ii) iron protoporphyrin IX covalently attached to a histidine residue in FixL (sensor protein in  Rhizobium nitrogen fixation pathway; ref.  26); ( iii) flavin adenine dinucleotide noncovalently bound to nitrogen fixation regulatory protein L and  Escherichia coli aerotaxis sensor ( 27-29); and ( iv) FMN noncovalently bound to phototropin ( 9,  12).	bind
29499	4	7382	7	NULL	NULL	0	NULL	flavin adenine dinucleotide 	NULL		bind	NULL	noncovalently			aerotaxis sensor	NULL	Escherichia coli 			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_6_2995_s_29	11248020	24 and  25); ( ii) iron protoporphyrin IX covalently attached to a histidine residue in FixL (sensor protein in  Rhizobium nitrogen fixation pathway; ref.  26); ( iii) flavin adenine dinucleotide noncovalently bound to nitrogen fixation regulatory protein L and  Escherichia coli aerotaxis sensor ( 27-29); and ( iv) FMN noncovalently bound to phototropin ( 9,  12).	bind
29500	5	7382	7	NULL	NULL	0	NULL	FMN	NULL		bind	NULL	noncovalently			phototropin	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_98_6_2995_s_29	11248020	24 and  25); ( ii) iron protoporphyrin IX covalently attached to a histidine residue in FixL (sensor protein in  Rhizobium nitrogen fixation pathway; ref.  26); ( iii) flavin adenine dinucleotide noncovalently bound to nitrogen fixation regulatory protein L and  Escherichia coli aerotaxis sensor ( 27-29); and ( iv) FMN noncovalently bound to phototropin ( 9,  12).	bind
27253	1	7383	5	13	NULL	NULL	NULL	VLDL E+	GP		transfered to					VLDL E-	GP	nascent			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_141	11557678	24 Another source of the apoE on VLDL could be from VLDL E+ transferring to nascent VLDL E-, although not so extensively as to produce a donor VLDL particle that no longerR binds to the anti-apoE column.	bind
27254	2	7383	5	13	NULL	NULL	NULL	statement 1	Process		is a source of					apoE	GP				NULL	VLDL	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_141	11557678	24 Another source of the apoE on VLDL could be from VLDL E+ transferring to nascent VLDL E-, although not so extensively as to produce a donor VLDL particle that no longerR binds to the anti-apoE column.	bind
29501	1	7383	7	NULL	NULL	0	NULL	VLDL E+	NULL		transfer to	NULL				VLDL E	NULL	nascent			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_141	11557678	24 Another source of the apoE on VLDL could be from VLDL E+ transferring to nascent VLDL E-, although not so extensively as to produce a donor VLDL particle that no longerR binds to the anti-apoE column.	bind
29503	2	7383	7	10	NULL	0	NULL	apoE VLDL			is from					statement 1					NULL	VLDL	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_141	11557678	24 Another source of the apoE on VLDL could be from VLDL E+ transferring to nascent VLDL E-, although not so extensively as to produce a donor VLDL particle that no longerR binds to the anti-apoE column.	bind
27336	1	7385	5	13	NULL	NULL	NULL	HBP/vigilin	GP		is associated with					t-RNA-protein complexes	GP	cytoplasmic			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2350_s_222	9409201	24 HBP/vigilin has also been found to be associated with cytoplasmic t-RNA-protein complexes isolated from human liver cells21 and from  Xenopus liver bound to vitellogenin mRNA.22 HBP/vigilin has also been reported to contain a functional nuclear localization sequence and to be present in the nucleus.	bind
27338	2	7385	5	13	NULL	NULL	NULL	t-RNA-protein complexes	GP	cytoplasmic	is isolated from					liver cells	Cell	human			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2350_s_222	9409201	24 HBP/vigilin has also been found to be associated with cytoplasmic t-RNA-protein complexes isolated from human liver cells21 and from  Xenopus liver bound to vitellogenin mRNA.22 HBP/vigilin has also been reported to contain a functional nuclear localization sequence and to be present in the nucleus.	bind
27341	3	7385	5	13	NULL	NULL	NULL	HBP/vigilin	GP		bind					vitellogenin mRNA	NucleicAcid				NULL	Xenopus liver	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2350_s_222	9409201	24 HBP/vigilin has also been found to be associated with cytoplasmic t-RNA-protein complexes isolated from human liver cells21 and from  Xenopus liver bound to vitellogenin mRNA.22 HBP/vigilin has also been reported to contain a functional nuclear localization sequence and to be present in the nucleus.	bind
27343	4	7385	5	13	NULL	NULL	NULL	HBP/vigilin	GP		contains							functional	nuclear localization sequence		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2350_s_222	9409201	24 HBP/vigilin has also been found to be associated with cytoplasmic t-RNA-protein complexes isolated from human liver cells21 and from  Xenopus liver bound to vitellogenin mRNA.22 HBP/vigilin has also been reported to contain a functional nuclear localization sequence and to be present in the nucleus.	bind
27344	5	7385	5	13	NULL	NULL	NULL	HBP/vigilin	GP		is present in					nucleus	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2350_s_222	9409201	24 HBP/vigilin has also been found to be associated with cytoplasmic t-RNA-protein complexes isolated from human liver cells21 and from  Xenopus liver bound to vitellogenin mRNA.22 HBP/vigilin has also been reported to contain a functional nuclear localization sequence and to be present in the nucleus.	bind
29506	1	7385	7	NULL	NULL	0	NULL	HBP/vigilin	NULL		associate with	NULL				 t-RNA-protein complexes 	NULL	cytoplasmic			NULL	human liver cells	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2350_s_222	9409201	24 HBP/vigilin has also been found to be associated with cytoplasmic t-RNA-protein complexes isolated from human liver cells21 and from  Xenopus liver bound to vitellogenin mRNA.22 HBP/vigilin has also been reported to contain a functional nuclear localization sequence and to be present in the nucleus.	bind
29507	2	7385	7	NULL	NULL	0	NULL	Xenopus liver	NULL		binds to	NULL				vitellogenin mRNA	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2350_s_222	9409201	24 HBP/vigilin has also been found to be associated with cytoplasmic t-RNA-protein complexes isolated from human liver cells21 and from  Xenopus liver bound to vitellogenin mRNA.22 HBP/vigilin has also been reported to contain a functional nuclear localization sequence and to be present in the nucleus.	bind
29508	3	7385	7	NULL	NULL	0	NULL	HBP/vigilin	NULL		associate with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2350_s_222	9409201	24 HBP/vigilin has also been found to be associated with cytoplasmic t-RNA-protein complexes isolated from human liver cells21 and from  Xenopus liver bound to vitellogenin mRNA.22 HBP/vigilin has also been reported to contain a functional nuclear localization sequence and to be present in the nucleus.	bind
29509	4	7385	7	NULL	NULL	0	NULL	HBP/vigilin	NULL		contains	NULL				functional nuclear localization sequence	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2350_s_222	9409201	24 HBP/vigilin has also been found to be associated with cytoplasmic t-RNA-protein complexes isolated from human liver cells21 and from  Xenopus liver bound to vitellogenin mRNA.22 HBP/vigilin has also been reported to contain a functional nuclear localization sequence and to be present in the nucleus.	bind
29510	5	7385	7	NULL	NULL	0	NULL	HBP/vigilin	NULL		is present in the 	NULL				nucleus	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2350_s_222	9409201	24 HBP/vigilin has also been found to be associated with cytoplasmic t-RNA-protein complexes isolated from human liver cells21 and from  Xenopus liver bound to vitellogenin mRNA.22 HBP/vigilin has also been reported to contain a functional nuclear localization sequence and to be present in the nucleus.	bind
27346	1	7386	5	13	NULL	NULL	NULL	Hp	GP		is found in		normally			serum	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_11_1193_s_214	12750308	24 Hp is normally found in serum in a >400 molar excess compared with free Hb, 25 and therefore all intravascular free Hb will be rapidly bound by Hp, preventing Hb-induced oxidation.	bind
27348	2	7386	5	13	NULL	NULL	NULL	Hb	GP	free	is found in					serum	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_11_1193_s_214	12750308	24 Hp is normally found in serum in a >400 molar excess compared with free Hb, 25 and therefore all intravascular free Hb will be rapidly bound by Hp, preventing Hb-induced oxidation.	bind
27349	3	7386	5	13	NULL	NULL	NULL	statement 1	GP		is more abundant than					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_11_1193_s_214	12750308	24 Hp is normally found in serum in a >400 molar excess compared with free Hb, 25 and therefore all intravascular free Hb will be rapidly bound by Hp, preventing Hb-induced oxidation.	bind
27350	4	7386	5	13	NULL	NULL	NULL	Hb	GP	intravascular free	bind		rapidly			Hp	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_11_1193_s_214	12750308	24 Hp is normally found in serum in a >400 molar excess compared with free Hb, 25 and therefore all intravascular free Hb will be rapidly bound by Hp, preventing Hb-induced oxidation.	bind
27351	5	7386	5	13	NULL	NULL	NULL	Hb	GP		induces					oxidation	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_11_1193_s_214	12750308	24 Hp is normally found in serum in a >400 molar excess compared with free Hb, 25 and therefore all intravascular free Hb will be rapidly bound by Hp, preventing Hb-induced oxidation.	bind
54484	6	7386	5	13	NULL	NULL	NULL	statement 4	Process		prevents					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_11_1193_s_214	12750308	24 Hp is normally found in serum in a >400 molar excess compared with free Hb, 25 and therefore all intravascular free Hb will be rapidly bound by Hp, preventing Hb-induced oxidation.	bind
29511	1	7386	7	10	NULL	0	NULL	Hp			is found in		normally			serum					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_11_1193_s_214	12750308	24 Hp is normally found in serum in a >400 molar excess compared with free Hb, 25 and therefore all intravascular free Hb will be rapidly bound by Hp, preventing Hb-induced oxidation.	bind
29512	2	7386	7	NULL	NULL	0	NULL	Hp	NULL		bind	NULL	rapidly			Hb	NULL	intravascular free			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_11_1193_s_214	12750308	24 Hp is normally found in serum in a >400 molar excess compared with free Hb, 25 and therefore all intravascular free Hb will be rapidly bound by Hp, preventing Hb-induced oxidation.	bind
29513	3	7386	7	NULL	NULL	0	NULL	Hb	NULL		induce	NULL				oxidation	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_92_11_1193_s_214	12750308	24 Hp is normally found in serum in a >400 molar excess compared with free Hb, 25 and therefore all intravascular free Hb will be rapidly bound by Hp, preventing Hb-induced oxidation.	bind
29514	4	7386	7	NULL	NULL	0	NULL	statement 2	NULL		prevents	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_92_11_1193_s_214	12750308	24 Hp is normally found in serum in a >400 molar excess compared with free Hb, 25 and therefore all intravascular free Hb will be rapidly bound by Hp, preventing Hb-induced oxidation.	bind
54485	5	7386	7	10	NULL	0	NULL	Hb		free	is found in					serum					NULL		0	NULL	NULL	NULL	gw60_circulationres_92_11_1193_s_214	12750308	24 Hp is normally found in serum in a >400 molar excess compared with free Hb, 25 and therefore all intravascular free Hb will be rapidly bound by Hp, preventing Hb-induced oxidation.	bind
54486	6	7386	7	10	NULL	0	NULL	statement 1			is more abundant than					statement 2					NULL		0	NULL	NULL	NULL	gw60_circulationres_92_11_1193_s_214	12750308	24 Hp is normally found in serum in a >400 molar excess compared with free Hb, 25 and therefore all intravascular free Hb will be rapidly bound by Hp, preventing Hb-induced oxidation.	bind
27356	1	7387	5	13	NULL	NULL	NULL	PPRE	NucleicAcid		is					PPAR response elements	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_546_s_32	10073956	24 Once activated, PPARgamma binds to the PPAR response elements (PPRE) in the promotor region of target genes.	bind
27358	2	7387	5	13	NULL	NULL	NULL	PPARgamma	GP	activated	bind					target genes	GP			PPRE in promoter	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_546_s_32	10073956	24 Once activated, PPARgamma binds to the PPAR response elements (PPRE) in the promotor region of target genes.	bind
29613	1	7387	7	10	NULL	0	NULL	PPARgamma		activated	binds to					target gene				PPRE in promoter	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_546_s_32	10073956	24 Once activated, PPARgamma binds to the PPAR response elements (PPRE) in the promotor region of target genes.	bind
29614	2	7387	7	NULL	NULL	0	NULL	PPRE	NULL		is	NULL				PPAR response elements	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_546_s_32	10073956	24 Once activated, PPARgamma binds to the PPAR response elements (PPRE) in the promotor region of target genes.	bind
27359	1	7388	5	13	NULL	NULL	NULL	SRE-1	NucleicAcid		bind					SREBP-1a	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_24_3104_s_25	12473559	24 SRE-1 can bind 3 different transcription factors: SREBP-1a, SREBP-1c, and SREBP-2.	bind
27360	2	7388	5	13	NULL	NULL	NULL	SRE-1	NucleicAcid		bind					SREBP-1c	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_24_3104_s_25	12473559	24 SRE-1 can bind 3 different transcription factors: SREBP-1a, SREBP-1c, and SREBP-2.	bind
27361	3	7388	5	13	NULL	NULL	NULL	SRE-1	NucleicAcid		bind					SREBP-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_24_3104_s_25	12473559	24 SRE-1 can bind 3 different transcription factors: SREBP-1a, SREBP-1c, and SREBP-2.	bind
29615	1	7388	7	NULL	NULL	0	NULL	 SRE-1	NULL		bind	NULL				SREBP-1a	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_24_3104_s_25	12473559	24 SRE-1 can bind 3 different transcription factors: SREBP-1a, SREBP-1c, and SREBP-2.	bind
29616	2	7388	7	NULL	NULL	0	NULL	SRE-1	NULL		bind	NULL				 SREBP-1c	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_24_3104_s_25	12473559	24 SRE-1 can bind 3 different transcription factors: SREBP-1a, SREBP-1c, and SREBP-2.	bind
29617	3	7388	7	NULL	NULL	0	NULL	SRE-1	NULL		bind	NULL				SREBP-2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_24_3104_s_25	12473559	24 SRE-1 can bind 3 different transcription factors: SREBP-1a, SREBP-1c, and SREBP-2.	bind
27363	1	7389	5	13	NULL	NULL	NULL	synthetic peptides	GP		contains					9 contiguous arginine residues	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1549_s_61	15231514	24 Synthetic peptides containing 9 contiguous arginine residues bind heparin with affinity similar to that of heparin-binding proteins.	bind
27364	2	7389	5	13	NULL	NULL	NULL	statement 1	GP		bind					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1549_s_61	15231514	24 Synthetic peptides containing 9 contiguous arginine residues bind heparin with affinity similar to that of heparin-binding proteins.	bind
27365	3	7389	5	13	NULL	NULL	NULL	statement 1	GP		bind					heparin-binding proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1549_s_61	15231514	24 Synthetic peptides containing 9 contiguous arginine residues bind heparin with affinity similar to that of heparin-binding proteins.	bind
27367	4	7389	5	13	NULL	NULL	NULL	statement 2	Process		similar affinity as					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1549_s_61	15231514	24 Synthetic peptides containing 9 contiguous arginine residues bind heparin with affinity similar to that of heparin-binding proteins.	bind
29618	2	7389	7	10	NULL	0	NULL	statement 1	NULL		bind	NULL				heparin	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1549_s_61	15231514	24 Synthetic peptides containing 9 contiguous arginine residues bind heparin with affinity similar to that of heparin-binding proteins.	bind
29619	3	7389	7	10	NULL	0	NULL	statement 1	NULL		bind	NULL				heparin-binding proteins	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1549_s_61	15231514	24 Synthetic peptides containing 9 contiguous arginine residues bind heparin with affinity similar to that of heparin-binding proteins.	bind
46603	1	7389	7	10	NULL	0	NULL	sythetic peptides 	NULL		contain	NULL				9 contiguous arginine residues	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1549_s_61	15231514	24 Synthetic peptides containing 9 contiguous arginine residues bind heparin with affinity similar to that of heparin-binding proteins.	bind
46604	4	7389	7	10	NULL	0	NULL	statement 2	NULL		is similar to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1549_s_61	15231514	24 Synthetic peptides containing 9 contiguous arginine residues bind heparin with affinity similar to that of heparin-binding proteins.	bind
27369	1	7390	5	13	NULL	NULL	NULL	P300	GP		bind									CRE/E-box complex	NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_23_2760_s_125	12057991	24 We determined P300 binding to the CRE/E-box complex.	bind
29620	1	7390	7	NULL	NULL	0	NULL	P300	NULL		binds to	NULL					NULL			CRE/E-box complex	NULL		0	NULL	NULL	NULL	gw60_circulation_105_23_2760_s_125	12057991	24 We determined P300 binding to the CRE/E-box complex.	bind
27373	1	7391	5	13	NULL	NULL	NULL	GFP-FRNK	GP		bind		competitively	C-terminal FAT sequence		paxillin	GP				NULL	NRVMs overexpressing GFP-FRNK	NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1282_s_219	12089066	24 We now show that in NRVMs overexpressing GFP-FRNK, FAK was displaced from focal adhesions, which was likely the result of competitive binding of GFP-FRNK to paxillin and other cytoskeletal proteins via its identical C-terminal FAT sequence.	bind
27375	2	7391	5	13	NULL	NULL	NULL	GFP-FRNK	GP		bind		competitively	C-terminal FAT sequence		cytoskeletal proteins	GP				NULL	NRVMs overexpressing GFP-FRNK	NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1282_s_219	12089066	24 We now show that in NRVMs overexpressing GFP-FRNK, FAK was displaced from focal adhesions, which was likely the result of competitive binding of GFP-FRNK to paxillin and other cytoskeletal proteins via its identical C-terminal FAT sequence.	bind
27379	3	7391	5	13	NULL	NULL	NULL	FAK	GP		is displaced from					focal adhesions	CellComponent				NULL	NRVMs overexpressing GFP-FRNK	NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1282_s_219	12089066	24 We now show that in NRVMs overexpressing GFP-FRNK, FAK was displaced from focal adhesions, which was likely the result of competitive binding of GFP-FRNK to paxillin and other cytoskeletal proteins via its identical C-terminal FAT sequence.	bind
27386	4	7391	5	13	NULL	NULL	NULL	statement 1	Process		results in		likely			statement 3	Process				NULL	NRVMs overexpressing GFP-FRNK	NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1282_s_219	12089066	24 We now show that in NRVMs overexpressing GFP-FRNK, FAK was displaced from focal adhesions, which was likely the result of competitive binding of GFP-FRNK to paxillin and other cytoskeletal proteins via its identical C-terminal FAT sequence.	bind
27388	5	7391	5	13	NULL	NULL	NULL	statement 2	Process		results in		likely			statement 3	Process				NULL	NRVMs overexpressing GFP-FRNK	NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1282_s_219	12089066	24 We now show that in NRVMs overexpressing GFP-FRNK, FAK was displaced from focal adhesions, which was likely the result of competitive binding of GFP-FRNK to paxillin and other cytoskeletal proteins via its identical C-terminal FAT sequence.	bind
29621	1	7391	7	NULL	NULL	0	NULL	 GFP-FRNK	NULL		bind	NULL		C-terminal FAT sequence		 paxillin	NULL				NULL	NRVMs overexpressing GFP-FRNK	NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1282_s_219	12089066	24 We now show that in NRVMs overexpressing GFP-FRNK, FAK was displaced from focal adhesions, which was likely the result of competitive binding of GFP-FRNK to paxillin and other cytoskeletal proteins via its identical C-terminal FAT sequence.	bind
29622	2	7391	7	NULL	NULL	0	NULL	GFP-FRNK	NULL		bind	NULL		C-terminal FAT sequence		cytoskeletal proteins	NULL				NULL	NRVMs overexpressing GFP-FRNK	NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1282_s_219	12089066	24 We now show that in NRVMs overexpressing GFP-FRNK, FAK was displaced from focal adhesions, which was likely the result of competitive binding of GFP-FRNK to paxillin and other cytoskeletal proteins via its identical C-terminal FAT sequence.	bind
29623	3	7391	7	10	NULL	0	NULL	FAK			displaced from					focal adhesions					NULL	NRVMs overexpressing GFP-FRNK	NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1282_s_219	12089066	24 We now show that in NRVMs overexpressing GFP-FRNK, FAK was displaced from focal adhesions, which was likely the result of competitive binding of GFP-FRNK to paxillin and other cytoskeletal proteins via its identical C-terminal FAT sequence.	bind
29624	4	7391	7	10	NULL	0	NULL	statement 1			leads to					statement 3					NULL	NRVMs overexpressing GFP-FRNK	NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1282_s_219	12089066	24 We now show that in NRVMs overexpressing GFP-FRNK, FAK was displaced from focal adhesions, which was likely the result of competitive binding of GFP-FRNK to paxillin and other cytoskeletal proteins via its identical C-terminal FAT sequence.	bind
29625	5	7391	7	10	NULL	0	NULL	statement 2			leads to					statement 3					NULL	NRVMs overexpressing GFP-FRNK	NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1282_s_219	12089066	24 We now show that in NRVMs overexpressing GFP-FRNK, FAK was displaced from focal adhesions, which was likely the result of competitive binding of GFP-FRNK to paxillin and other cytoskeletal proteins via its identical C-terminal FAT sequence.	bind
27394	1	7392	5	13	NULL	NULL	NULL	CD40L	GP		is					CD40 ligand	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_1_229_s_21	9916937	24, 25  CD40 binds CD40 ligand (CD40L, also referred to as gp39 or TRAP), a cell surface molecule until recently considered restricted to activated CD4+ T cells.	bind
27396	2	7392	5	13	NULL	NULL	NULL	CD40L	GP		is a synonym of					gp39	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_1_229_s_21	9916937	24, 25  CD40 binds CD40 ligand (CD40L, also referred to as gp39 or TRAP), a cell surface molecule until recently considered restricted to activated CD4+ T cells.	bind
27397	3	7392	5	13	NULL	NULL	NULL	CD40L	GP		is a synonym of					TRAP	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_1_229_s_21	9916937	24, 25  CD40 binds CD40 ligand (CD40L, also referred to as gp39 or TRAP), a cell surface molecule until recently considered restricted to activated CD4+ T cells.	bind
27398	4	7392	5	13	NULL	NULL	NULL	statement 2	GP		is an alternative to					statement 3	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_1_229_s_21	9916937	24, 25  CD40 binds CD40 ligand (CD40L, also referred to as gp39 or TRAP), a cell surface molecule until recently considered restricted to activated CD4+ T cells.	bind
27400	5	7392	5	13	NULL	NULL	NULL	 CD40	GP		bind					CD40L	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_1_229_s_21	9916937	24, 25  CD40 binds CD40 ligand (CD40L, also referred to as gp39 or TRAP), a cell surface molecule until recently considered restricted to activated CD4+ T cells.	bind
27401	6	7392	5	13	NULL	NULL	NULL	CD40L	GP		is a type of					cell surface molecule	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_1_229_s_21	9916937	24, 25  CD40 binds CD40 ligand (CD40L, also referred to as gp39 or TRAP), a cell surface molecule until recently considered restricted to activated CD4+ T cells.	bind
27402	7	7392	5	13	NULL	NULL	NULL	CD40L	GP		is restricted to					CD4+ T cells	Cell	activated			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_1_229_s_21	9916937	24, 25  CD40 binds CD40 ligand (CD40L, also referred to as gp39 or TRAP), a cell surface molecule until recently considered restricted to activated CD4+ T cells.	bind
29626	1	7392	7	NULL	NULL	0	NULL	CD40 	NULL		binds	NULL				CD40L	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_1_229_s_21	9916937	24, 25  CD40 binds CD40 ligand (CD40L, also referred to as gp39 or TRAP), a cell surface molecule until recently considered restricted to activated CD4+ T cells.	bind
29627	2	7392	7	NULL	NULL	0	NULL	CD40L	NULL		is	NULL				CD40 ligand	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_1_229_s_21	9916937	24, 25  CD40 binds CD40 ligand (CD40L, also referred to as gp39 or TRAP), a cell surface molecule until recently considered restricted to activated CD4+ T cells.	bind
29628	3	7392	7	10	NULL	0	NULL	CD40			is a synonym of					gp39					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_1_229_s_21	9916937	24, 25  CD40 binds CD40 ligand (CD40L, also referred to as gp39 or TRAP), a cell surface molecule until recently considered restricted to activated CD4+ T cells.	bind
29629	4	7392	7	10	NULL	0	NULL	CD40L			is a synonym of					TRAP					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_1_229_s_21	9916937	24, 25  CD40 binds CD40 ligand (CD40L, also referred to as gp39 or TRAP), a cell surface molecule until recently considered restricted to activated CD4+ T cells.	bind
29630	5	7392	7	NULL	NULL	0	NULL	CD40L 	NULL		is a type of	NULL				cell surface molecule	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_1_229_s_21	9916937	24, 25  CD40 binds CD40 ligand (CD40L, also referred to as gp39 or TRAP), a cell surface molecule until recently considered restricted to activated CD4+ T cells.	bind
29631	6	7392	7	NULL	NULL	0	NULL	CD40L	NULL		is restricted to	NULL				CD4+ T cells	NULL	activated			NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_1_229_s_21	9916937	24, 25  CD40 binds CD40 ligand (CD40L, also referred to as gp39 or TRAP), a cell surface molecule until recently considered restricted to activated CD4+ T cells.	bind
27405	1	7393	5	13	NULL	NULL	NULL	FAP-1	GP		promote		may			Fas resistance	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_4_1335_s_224	11290551	24, 25  In addition, whereas FAP-1 may promote Fas resistance in some cell types, deletion of the C-terminal FAP-1-binding region of Fas did not alter its ability to induce apoptosis in murine lymphoid cell lines, implying that the relative importance of FAP-1 as an inhibitor of Fas-induced apoptosis may be dependent on cell context.	bind
27407	2	7393	5	13	NULL	NULL	NULL				is deleted from			C-terminal FAP-1-binding region		Fas	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_4_1335_s_224	11290551	24, 25  In addition, whereas FAP-1 may promote Fas resistance in some cell types, deletion of the C-terminal FAP-1-binding region of Fas did not alter its ability to induce apoptosis in murine lymphoid cell lines, implying that the relative importance of FAP-1 as an inhibitor of Fas-induced apoptosis may be dependent on cell context.	bind
27409	3	7393	5	13	NULL	NULL	NULL	Fas	GP		induces					apoptosis	Process				NULL	in murine lymphoid cell lines	NULL	NULL	NULL	NULL	gw60_amjpathol_158_4_1335_s_224	11290551	24, 25  In addition, whereas FAP-1 may promote Fas resistance in some cell types, deletion of the C-terminal FAP-1-binding region of Fas did not alter its ability to induce apoptosis in murine lymphoid cell lines, implying that the relative importance of FAP-1 as an inhibitor of Fas-induced apoptosis may be dependent on cell context.	bind
27410	4	7393	5	13	NULL	NULL	NULL	statement 2	Process		does not alter					statement 3	Process	ability of			NULL	in murine lymphoid cell lines	NULL	NULL	NULL	NULL	gw60_amjpathol_158_4_1335_s_224	11290551	24, 25  In addition, whereas FAP-1 may promote Fas resistance in some cell types, deletion of the C-terminal FAP-1-binding region of Fas did not alter its ability to induce apoptosis in murine lymphoid cell lines, implying that the relative importance of FAP-1 as an inhibitor of Fas-induced apoptosis may be dependent on cell context.	bind
27411	5	7393	5	13	NULL	NULL	NULL	FAP-1	GP		is inhibitor of					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_4_1335_s_224	11290551	24, 25  In addition, whereas FAP-1 may promote Fas resistance in some cell types, deletion of the C-terminal FAP-1-binding region of Fas did not alter its ability to induce apoptosis in murine lymphoid cell lines, implying that the relative importance of FAP-1 as an inhibitor of Fas-induced apoptosis may be dependent on cell context.	bind
27412	6	7393	5	13	NULL	NULL	NULL	statement 5	Process	importance of	is dependent on					cell context	Cell				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_4_1335_s_224	11290551	24, 25  In addition, whereas FAP-1 may promote Fas resistance in some cell types, deletion of the C-terminal FAP-1-binding region of Fas did not alter its ability to induce apoptosis in murine lymphoid cell lines, implying that the relative importance of FAP-1 as an inhibitor of Fas-induced apoptosis may be dependent on cell context.	bind
27413	7	7393	5	13	NULL	NULL	NULL	statement 4	Process		imply					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_4_1335_s_224	11290551	24, 25  In addition, whereas FAP-1 may promote Fas resistance in some cell types, deletion of the C-terminal FAP-1-binding region of Fas did not alter its ability to induce apoptosis in murine lymphoid cell lines, implying that the relative importance of FAP-1 as an inhibitor of Fas-induced apoptosis may be dependent on cell context.	bind
29632	1	7393	7	NULL	NULL	0	NULL	FAP-1	NULL		promote	NULL	may			Fas resistance	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_4_1335_s_224	11290551	24, 25  In addition, whereas FAP-1 may promote Fas resistance in some cell types, deletion of the C-terminal FAP-1-binding region of Fas did not alter its ability to induce apoptosis in murine lymphoid cell lines, implying that the relative importance of FAP-1 as an inhibitor of Fas-induced apoptosis may be dependent on cell context.	bind
29633	2	7393	7	NULL	NULL	0	NULL	Fas	NULL	deletion of	does not alter	NULL		C-terminal FAP-1-binding region		apoptosis	NULL	its ability to induce			NULL	murine lymphoid cell lines	NULL	NULL	NULL	NULL	gw60_amjpathol_158_4_1335_s_224	11290551	24, 25  In addition, whereas FAP-1 may promote Fas resistance in some cell types, deletion of the C-terminal FAP-1-binding region of Fas did not alter its ability to induce apoptosis in murine lymphoid cell lines, implying that the relative importance of FAP-1 as an inhibitor of Fas-induced apoptosis may be dependent on cell context.	bind
29634	3	7393	7	NULL	NULL	0	NULL	 Fas	NULL		induce	NULL				apoptosis	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_4_1335_s_224	11290551	24, 25  In addition, whereas FAP-1 may promote Fas resistance in some cell types, deletion of the C-terminal FAP-1-binding region of Fas did not alter its ability to induce apoptosis in murine lymphoid cell lines, implying that the relative importance of FAP-1 as an inhibitor of Fas-induced apoptosis may be dependent on cell context.	bind
29635	4	7393	7	NULL	NULL	0	NULL	 FAP-1	NULL		inhibits	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_4_1335_s_224	11290551	24, 25  In addition, whereas FAP-1 may promote Fas resistance in some cell types, deletion of the C-terminal FAP-1-binding region of Fas did not alter its ability to induce apoptosis in murine lymphoid cell lines, implying that the relative importance of FAP-1 as an inhibitor of Fas-induced apoptosis may be dependent on cell context.	bind
29636	5	7393	7	NULL	NULL	0	NULL	statement 4	NULL		depends on	NULL				cell context	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_4_1335_s_224	11290551	24, 25  In addition, whereas FAP-1 may promote Fas resistance in some cell types, deletion of the C-terminal FAP-1-binding region of Fas did not alter its ability to induce apoptosis in murine lymphoid cell lines, implying that the relative importance of FAP-1 as an inhibitor of Fas-induced apoptosis may be dependent on cell context.	bind
27414	1	7394	5	13	NULL	NULL	NULL	insulin receptor	GP		bind		high affinity			insulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_5_1905_s_282	11696451	24, 25  The insulin receptor demonstrates high-affinity binding to insulin and lower affinity binding to IGF-1, whereas the IGF-1 receptor binds IGF-1 (and IGF-2) with a higher affinity than it does insulin.	bind
27415	2	7394	5	13	NULL	NULL	NULL	insulin receptor	GP		bind		low affinity			IGF-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_5_1905_s_282	11696451	24, 25  The insulin receptor demonstrates high-affinity binding to insulin and lower affinity binding to IGF-1, whereas the IGF-1 receptor binds IGF-1 (and IGF-2) with a higher affinity than it does insulin.	bind
27416	3	7394	5	13	NULL	NULL	NULL	IGF-1 receptor	GP		bind					IGF-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_5_1905_s_282	11696451	24, 25  The insulin receptor demonstrates high-affinity binding to insulin and lower affinity binding to IGF-1, whereas the IGF-1 receptor binds IGF-1 (and IGF-2) with a higher affinity than it does insulin.	bind
27417	4	7394	5	13	NULL	NULL	NULL	IGF-1 receptor	GP		bind					IGF-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_5_1905_s_282	11696451	24, 25  The insulin receptor demonstrates high-affinity binding to insulin and lower affinity binding to IGF-1, whereas the IGF-1 receptor binds IGF-1 (and IGF-2) with a higher affinity than it does insulin.	bind
27418	5	7394	5	13	NULL	NULL	NULL	IGF-1 receptor	GP		bind					insulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_5_1905_s_282	11696451	24, 25  The insulin receptor demonstrates high-affinity binding to insulin and lower affinity binding to IGF-1, whereas the IGF-1 receptor binds IGF-1 (and IGF-2) with a higher affinity than it does insulin.	bind
27419	6	7394	5	13	NULL	NULL	NULL	statement 3	Process		has high affinity than					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_5_1905_s_282	11696451	24, 25  The insulin receptor demonstrates high-affinity binding to insulin and lower affinity binding to IGF-1, whereas the IGF-1 receptor binds IGF-1 (and IGF-2) with a higher affinity than it does insulin.	bind
27420	7	7394	5	13	NULL	NULL	NULL	statement 4	Process		has high affinity than					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_5_1905_s_282	11696451	24, 25  The insulin receptor demonstrates high-affinity binding to insulin and lower affinity binding to IGF-1, whereas the IGF-1 receptor binds IGF-1 (and IGF-2) with a higher affinity than it does insulin.	bind
29637	1	7394	7	NULL	NULL	0	NULL	insulin receptor	NULL		bind	NULL	high-affinity			insulin	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_5_1905_s_282	11696451	24, 25  The insulin receptor demonstrates high-affinity binding to insulin and lower affinity binding to IGF-1, whereas the IGF-1 receptor binds IGF-1 (and IGF-2) with a higher affinity than it does insulin.	bind
29638	2	7394	7	NULL	NULL	0	NULL	insulin receptor	NULL		bind	NULL	low affinity			IGF-1	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_5_1905_s_282	11696451	24, 25  The insulin receptor demonstrates high-affinity binding to insulin and lower affinity binding to IGF-1, whereas the IGF-1 receptor binds IGF-1 (and IGF-2) with a higher affinity than it does insulin.	bind
29639	3	7394	7	NULL	NULL	0	NULL	IGF-1 receptor	NULL		binds	NULL				IGF-1 	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_5_1905_s_282	11696451	24, 25  The insulin receptor demonstrates high-affinity binding to insulin and lower affinity binding to IGF-1, whereas the IGF-1 receptor binds IGF-1 (and IGF-2) with a higher affinity than it does insulin.	bind
29640	4	7394	7	NULL	NULL	0	NULL	IGF-1 receptor	NULL		binds	NULL				IGF-2	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_5_1905_s_282	11696451	24, 25  The insulin receptor demonstrates high-affinity binding to insulin and lower affinity binding to IGF-1, whereas the IGF-1 receptor binds IGF-1 (and IGF-2) with a higher affinity than it does insulin.	bind
29641	5	7394	7	NULL	NULL	0	NULL	IGF-1 receptor	NULL		bind	NULL				insulin	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_5_1905_s_282	11696451	24, 25  The insulin receptor demonstrates high-affinity binding to insulin and lower affinity binding to IGF-1, whereas the IGF-1 receptor binds IGF-1 (and IGF-2) with a higher affinity than it does insulin.	bind
29642	6	7394	7	NULL	NULL	0	NULL	statement 3	NULL		has higher affinity than	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_5_1905_s_282	11696451	24, 25  The insulin receptor demonstrates high-affinity binding to insulin and lower affinity binding to IGF-1, whereas the IGF-1 receptor binds IGF-1 (and IGF-2) with a higher affinity than it does insulin.	bind
29643	7	7394	7	NULL	NULL	0	NULL	statement 4	NULL		has higher affinity than	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_5_1905_s_282	11696451	24, 25  The insulin receptor demonstrates high-affinity binding to insulin and lower affinity binding to IGF-1, whereas the IGF-1 receptor binds IGF-1 (and IGF-2) with a higher affinity than it does insulin.	bind
27421	1	7395	5	13	NULL	NULL	NULL	ATP	Chemical		is hydrolysed to					ADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_89_3_279_s_220	11485979	24, 25 After hydrolysis of ATP to ADP, cytochrome  c binds to Apaf-1, promoting its multimerization from a monomeric form to a large complex.	bind
27422	2	7395	5	13	NULL	NULL	NULL	cytochrome c	GP		bind					Apaf-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_89_3_279_s_220	11485979	24, 25 After hydrolysis of ATP to ADP, cytochrome  c binds to Apaf-1, promoting its multimerization from a monomeric form to a large complex.	bind
27423	3	7395	5	13	NULL	NULL	NULL	statement 2	Process		occurs after					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_89_3_279_s_220	11485979	24, 25 After hydrolysis of ATP to ADP, cytochrome  c binds to Apaf-1, promoting its multimerization from a monomeric form to a large complex.	bind
27424	4	7395	5	13	NULL	NULL	NULL	Apaf-1 monomer	GP		multimerize to					large complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_89_3_279_s_220	11485979	24, 25 After hydrolysis of ATP to ADP, cytochrome  c binds to Apaf-1, promoting its multimerization from a monomeric form to a large complex.	bind
27425	5	7395	5	13	NULL	NULL	NULL	statement 2	Process		promote					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_89_3_279_s_220	11485979	24, 25 After hydrolysis of ATP to ADP, cytochrome  c binds to Apaf-1, promoting its multimerization from a monomeric form to a large complex.	bind
29644	1	7395	7	NULL	NULL	0	NULL	cytochrome c	NULL		binds to	NULL				Apaf-1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_89_3_279_s_220	11485979	24, 25 After hydrolysis of ATP to ADP, cytochrome  c binds to Apaf-1, promoting its multimerization from a monomeric form to a large complex.	bind
29645	2	7395	7	NULL	NULL	0	NULL	ATP	NULL		hydrolysed to	NULL				ADP	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_89_3_279_s_220	11485979	24, 25 After hydrolysis of ATP to ADP, cytochrome  c binds to Apaf-1, promoting its multimerization from a monomeric form to a large complex.	bind
29646	3	7395	7	NULL	NULL	0	NULL	statement 1	NULL		occurs after	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_89_3_279_s_220	11485979	24, 25 After hydrolysis of ATP to ADP, cytochrome  c binds to Apaf-1, promoting its multimerization from a monomeric form to a large complex.	bind
29647	4	7395	7	10	NULL	0	NULL	Apaf-1 monomer			multimerizes to					large complex					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_89_3_279_s_220	11485979	24, 25 After hydrolysis of ATP to ADP, cytochrome  c binds to Apaf-1, promoting its multimerization from a monomeric form to a large complex.	bind
29648	5	7395	7	NULL	NULL	0	NULL	statement 1	NULL		promotes	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_89_3_279_s_220	11485979	24, 25 After hydrolysis of ATP to ADP, cytochrome  c binds to Apaf-1, promoting its multimerization from a monomeric form to a large complex.	bind
27426	1	7396	5	13	NULL	NULL	NULL	apoA-I	GP		bind					integral membrane protein	GP				NULL	in ABCA1-expressing cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_40	12738681	24,25  Using a fluorescence photobleaching technique, this study also suggested that apoA-I bound to an integral membrane protein in ABCA1-expressing cells.	bind
29649	1	7396	7	NULL	NULL	0	NULL	apoA-I	NULL		bind	NULL				integral membrane protein	NULL				NULL	ABCA1-expressing cells	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_40	12738681	24,25  Using a fluorescence photobleaching technique, this study also suggested that apoA-I bound to an integral membrane protein in ABCA1-expressing cells.	bind
27427	1	7397	5	13	NULL	NULL	NULL	ETF	GP		bind					p53	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_34_23777_s_233	10446138	243R Is Required for the Binding of both ETF and E2F to the p53 Promoter-- Both E1a proteins, 243R and 289R, are transcriptional activators; however, they are thought to bring about activation by different mechanisms ( 38,  77,  80).	bind
27428	2	7397	5	13	NULL	NULL	NULL	E2F	GP		bind					p53	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_34_23777_s_233	10446138	243R Is Required for the Binding of both ETF and E2F to the p53 Promoter-- Both E1a proteins, 243R and 289R, are transcriptional activators; however, they are thought to bring about activation by different mechanisms ( 38,  77,  80).	bind
27429	3	7397	5	13	NULL	NULL	NULL	243R	GP		is required for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_34_23777_s_233	10446138	243R Is Required for the Binding of both ETF and E2F to the p53 Promoter-- Both E1a proteins, 243R and 289R, are transcriptional activators; however, they are thought to bring about activation by different mechanisms ( 38,  77,  80).	bind
27430	4	7397	5	13	NULL	NULL	NULL	243R	GP		is required for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_34_23777_s_233	10446138	243R Is Required for the Binding of both ETF and E2F to the p53 Promoter-- Both E1a proteins, 243R and 289R, are transcriptional activators; however, they are thought to bring about activation by different mechanisms ( 38,  77,  80).	bind
27431	5	7397	5	13	NULL	NULL	NULL	243R	GP		is a type of					E1a proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_34_23777_s_233	10446138	243R Is Required for the Binding of both ETF and E2F to the p53 Promoter-- Both E1a proteins, 243R and 289R, are transcriptional activators; however, they are thought to bring about activation by different mechanisms ( 38,  77,  80).	bind
27432	6	7397	5	13	NULL	NULL	NULL	289R	GP		is a type of					E1a proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_34_23777_s_233	10446138	243R Is Required for the Binding of both ETF and E2F to the p53 Promoter-- Both E1a proteins, 243R and 289R, are transcriptional activators; however, they are thought to bring about activation by different mechanisms ( 38,  77,  80).	bind
27433	7	7397	5	13	NULL	NULL	NULL	243R	GP		function as					transcriptional activator	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_34_23777_s_233	10446138	243R Is Required for the Binding of both ETF and E2F to the p53 Promoter-- Both E1a proteins, 243R and 289R, are transcriptional activators; however, they are thought to bring about activation by different mechanisms ( 38,  77,  80).	bind
27434	8	7397	5	13	NULL	NULL	NULL	289R	GP		function as					transcriptional activator	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_34_23777_s_233	10446138	243R Is Required for the Binding of both ETF and E2F to the p53 Promoter-- Both E1a proteins, 243R and 289R, are transcriptional activators; however, they are thought to bring about activation by different mechanisms ( 38,  77,  80).	bind
27435	9	7397	5	13	NULL	NULL	NULL	243R	GP	mechanism of activation by	differs from					289R	GP	mechanism of activation by			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_34_23777_s_233	10446138	243R Is Required for the Binding of both ETF and E2F to the p53 Promoter-- Both E1a proteins, 243R and 289R, are transcriptional activators; however, they are thought to bring about activation by different mechanisms ( 38,  77,  80).	bind
29650	1	7397	7	NULL	NULL	0	NULL	ETF	NULL		bind	NULL				p53	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_34_23777_s_233	10446138	243R Is Required for the Binding of both ETF and E2F to the p53 Promoter-- Both E1a proteins, 243R and 289R, are transcriptional activators; however, they are thought to bring about activation by different mechanisms ( 38,  77,  80).	bind
29651	2	7397	7	NULL	NULL	0	NULL	E2F	NULL		bind	NULL				p53	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_34_23777_s_233	10446138	243R Is Required for the Binding of both ETF and E2F to the p53 Promoter-- Both E1a proteins, 243R and 289R, are transcriptional activators; however, they are thought to bring about activation by different mechanisms ( 38,  77,  80).	bind
29652	3	7397	7	NULL	NULL	0	NULL	243R	NULL		is required for	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_34_23777_s_233	10446138	243R Is Required for the Binding of both ETF and E2F to the p53 Promoter-- Both E1a proteins, 243R and 289R, are transcriptional activators; however, they are thought to bring about activation by different mechanisms ( 38,  77,  80).	bind
29653	4	7397	7	NULL	NULL	0	NULL	243R	NULL		is required for	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_34_23777_s_233	10446138	243R Is Required for the Binding of both ETF and E2F to the p53 Promoter-- Both E1a proteins, 243R and 289R, are transcriptional activators; however, they are thought to bring about activation by different mechanisms ( 38,  77,  80).	bind
29654	5	7397	7	NULL	NULL	0	NULL	243R	NULL		is a type of	NULL				transcriptional activator	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_34_23777_s_233	10446138	243R Is Required for the Binding of both ETF and E2F to the p53 Promoter-- Both E1a proteins, 243R and 289R, are transcriptional activators; however, they are thought to bring about activation by different mechanisms ( 38,  77,  80).	bind
29655	6	7397	7	NULL	NULL	0	NULL	289R	NULL		is a type of	NULL				transcriptional activator	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_34_23777_s_233	10446138	243R Is Required for the Binding of both ETF and E2F to the p53 Promoter-- Both E1a proteins, 243R and 289R, are transcriptional activators; however, they are thought to bring about activation by different mechanisms ( 38,  77,  80).	bind
29656	7	7397	7	NULL	NULL	0	NULL	243R	NULL		is a type of	NULL				E1a protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_34_23777_s_233	10446138	243R Is Required for the Binding of both ETF and E2F to the p53 Promoter-- Both E1a proteins, 243R and 289R, are transcriptional activators; however, they are thought to bring about activation by different mechanisms ( 38,  77,  80).	bind
29657	8	7397	7	NULL	NULL	0	NULL	289R	NULL		is a type of	NULL				E1a protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_34_23777_s_233	10446138	243R Is Required for the Binding of both ETF and E2F to the p53 Promoter-- Both E1a proteins, 243R and 289R, are transcriptional activators; however, they are thought to bring about activation by different mechanisms ( 38,  77,  80).	bind
27436	1	7398	5	13	NULL	NULL	NULL	24p3	GP		bind		specifically			statement 15	Cell				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5531_829_s_102	11486081	24p3 also bound specifically to IL-3-dependent primary bone marrow cells and to other leukocytic cell lines, such as 32D and murine HT-2, which are susceptible to 24p3-mediated apoptosis but not to nonhematopoietic cell lines, such as murine NIH 3T3 and COS-7, which are resistant.	bind
27437	2	7398	5	13	NULL	NULL	NULL	24p3	GP		bind		specifically			32D	Cell				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5531_829_s_102	11486081	24p3 also bound specifically to IL-3-dependent primary bone marrow cells and to other leukocytic cell lines, such as 32D and murine HT-2, which are susceptible to 24p3-mediated apoptosis but not to nonhematopoietic cell lines, such as murine NIH 3T3 and COS-7, which are resistant.	bind
27438	3	7398	5	13	NULL	NULL	NULL	24p3	GP		bind		specifically			HT-2	Cell	murine			NULL		NULL	NULL	NULL	NULL	gw60_science_293_5531_829_s_102	11486081	24p3 also bound specifically to IL-3-dependent primary bone marrow cells and to other leukocytic cell lines, such as 32D and murine HT-2, which are susceptible to 24p3-mediated apoptosis but not to nonhematopoietic cell lines, such as murine NIH 3T3 and COS-7, which are resistant.	bind
27439	4	7398	5	13	NULL	NULL	NULL	32D	Cell		is a type of					leukocytic cell lines	Cell				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5531_829_s_102	11486081	24p3 also bound specifically to IL-3-dependent primary bone marrow cells and to other leukocytic cell lines, such as 32D and murine HT-2, which are susceptible to 24p3-mediated apoptosis but not to nonhematopoietic cell lines, such as murine NIH 3T3 and COS-7, which are resistant.	bind
27440	5	7398	5	13	NULL	NULL	NULL	HT-2	Cell	murine	is a type of					leukocytic cell lines	Cell				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5531_829_s_102	11486081	24p3 also bound specifically to IL-3-dependent primary bone marrow cells and to other leukocytic cell lines, such as 32D and murine HT-2, which are susceptible to 24p3-mediated apoptosis but not to nonhematopoietic cell lines, such as murine NIH 3T3 and COS-7, which are resistant.	bind
27441	6	7398	5	13	NULL	NULL	NULL	32D	Cell		is susceptible to					statement 14	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5531_829_s_102	11486081	24p3 also bound specifically to IL-3-dependent primary bone marrow cells and to other leukocytic cell lines, such as 32D and murine HT-2, which are susceptible to 24p3-mediated apoptosis but not to nonhematopoietic cell lines, such as murine NIH 3T3 and COS-7, which are resistant.	bind
27442	7	7398	5	13	NULL	NULL	NULL	HT-2	Cell	murine	is susceptible to					statement 14	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5531_829_s_102	11486081	24p3 also bound specifically to IL-3-dependent primary bone marrow cells and to other leukocytic cell lines, such as 32D and murine HT-2, which are susceptible to 24p3-mediated apoptosis but not to nonhematopoietic cell lines, such as murine NIH 3T3 and COS-7, which are resistant.	bind
27443	8	7398	5	13	NULL	NULL	NULL	NIH 3T3	Cell	murine	is a type of					nonhematopoietic cell lines	Cell				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5531_829_s_102	11486081	24p3 also bound specifically to IL-3-dependent primary bone marrow cells and to other leukocytic cell lines, such as 32D and murine HT-2, which are susceptible to 24p3-mediated apoptosis but not to nonhematopoietic cell lines, such as murine NIH 3T3 and COS-7, which are resistant.	bind
27444	9	7398	5	13	NULL	NULL	NULL	COS-7	Cell		is a type of					nonhematopoietic cell lines	Cell				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5531_829_s_102	11486081	24p3 also bound specifically to IL-3-dependent primary bone marrow cells and to other leukocytic cell lines, such as 32D and murine HT-2, which are susceptible to 24p3-mediated apoptosis but not to nonhematopoietic cell lines, such as murine NIH 3T3 and COS-7, which are resistant.	bind
27445	10	7398	5	13	NULL	NULL	NULL	24p3	GP		does not bind					NIH 3T3	Cell	murine			NULL		NULL	NULL	NULL	NULL	gw60_science_293_5531_829_s_102	11486081	24p3 also bound specifically to IL-3-dependent primary bone marrow cells and to other leukocytic cell lines, such as 32D and murine HT-2, which are susceptible to 24p3-mediated apoptosis but not to nonhematopoietic cell lines, such as murine NIH 3T3 and COS-7, which are resistant.	bind
27446	11	7398	5	13	NULL	NULL	NULL	24p3	GP		does not bind					COS-7	Cell				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5531_829_s_102	11486081	24p3 also bound specifically to IL-3-dependent primary bone marrow cells and to other leukocytic cell lines, such as 32D and murine HT-2, which are susceptible to 24p3-mediated apoptosis but not to nonhematopoietic cell lines, such as murine NIH 3T3 and COS-7, which are resistant.	bind
27447	12	7398	5	13	NULL	NULL	NULL	NIH 3T3	Cell	murine	is resistant to					apoptosis	Process	24p3-mediated			NULL		NULL	NULL	NULL	NULL	gw60_science_293_5531_829_s_102	11486081	24p3 also bound specifically to IL-3-dependent primary bone marrow cells and to other leukocytic cell lines, such as 32D and murine HT-2, which are susceptible to 24p3-mediated apoptosis but not to nonhematopoietic cell lines, such as murine NIH 3T3 and COS-7, which are resistant.	bind
27448	13	7398	5	13	NULL	NULL	NULL	COS-7	Cell		is resistant to					apoptosis	Process	24p3-mediated			NULL		NULL	NULL	NULL	NULL	gw60_science_293_5531_829_s_102	11486081	24p3 also bound specifically to IL-3-dependent primary bone marrow cells and to other leukocytic cell lines, such as 32D and murine HT-2, which are susceptible to 24p3-mediated apoptosis but not to nonhematopoietic cell lines, such as murine NIH 3T3 and COS-7, which are resistant.	bind
54487	14	7398	5	13	NULL	NULL	NULL	24p3	GP		mediates					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5531_829_s_102	11486081	24p3 also bound specifically to IL-3-dependent primary bone marrow cells and to other leukocytic cell lines, such as 32D and murine HT-2, which are susceptible to 24p3-mediated apoptosis but not to nonhematopoietic cell lines, such as murine NIH 3T3 and COS-7, which are resistant.	bind
54488	15	7398	5	13	NULL	NULL	NULL	\tprimary bone marrow cells	Cell		is dependent on					IL-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5531_829_s_102	11486081	24p3 also bound specifically to IL-3-dependent primary bone marrow cells and to other leukocytic cell lines, such as 32D and murine HT-2, which are susceptible to 24p3-mediated apoptosis but not to nonhematopoietic cell lines, such as murine NIH 3T3 and COS-7, which are resistant.	bind
29658	1	7398	7	10	NULL	0	NULL	24p3			bind		specifically			statement 15					NULL		NULL	NULL	NULL	NULL	gw60_science_293_5531_829_s_102	11486081	24p3 also bound specifically to IL-3-dependent primary bone marrow cells and to other leukocytic cell lines, such as 32D and murine HT-2, which are susceptible to 24p3-mediated apoptosis but not to nonhematopoietic cell lines, such as murine NIH 3T3 and COS-7, which are resistant.	bind
29659	2	7398	7	NULL	NULL	0	NULL	24p3	NULL		bind	NULL	specifically			32D	NULL				NULL		0	NULL	NULL	NULL	gw60_science_293_5531_829_s_102	11486081	24p3 also bound specifically to IL-3-dependent primary bone marrow cells and to other leukocytic cell lines, such as 32D and murine HT-2, which are susceptible to 24p3-mediated apoptosis but not to nonhematopoietic cell lines, such as murine NIH 3T3 and COS-7, which are resistant.	bind
29660	3	7398	7	NULL	NULL	0	NULL	24p3	NULL		bind	NULL	specifically			HT-2	NULL	murine			NULL		0	NULL	NULL	NULL	gw60_science_293_5531_829_s_102	11486081	24p3 also bound specifically to IL-3-dependent primary bone marrow cells and to other leukocytic cell lines, such as 32D and murine HT-2, which are susceptible to 24p3-mediated apoptosis but not to nonhematopoietic cell lines, such as murine NIH 3T3 and COS-7, which are resistant.	bind
29661	4	7398	7	NULL	NULL	0	NULL	24p3	NULL		mediates	NULL				apoptosis	NULL				NULL		0	NULL	NULL	NULL	gw60_science_293_5531_829_s_102	11486081	24p3 also bound specifically to IL-3-dependent primary bone marrow cells and to other leukocytic cell lines, such as 32D and murine HT-2, which are susceptible to 24p3-mediated apoptosis but not to nonhematopoietic cell lines, such as murine NIH 3T3 and COS-7, which are resistant.	bind
29662	5	7398	7	NULL	NULL	0	NULL	32D	NULL		is susceptible to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_science_293_5531_829_s_102	11486081	24p3 also bound specifically to IL-3-dependent primary bone marrow cells and to other leukocytic cell lines, such as 32D and murine HT-2, which are susceptible to 24p3-mediated apoptosis but not to nonhematopoietic cell lines, such as murine NIH 3T3 and COS-7, which are resistant.	bind
29663	6	7398	7	NULL	NULL	0	NULL	HT-2	NULL	murine	is susceptible to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_science_293_5531_829_s_102	11486081	24p3 also bound specifically to IL-3-dependent primary bone marrow cells and to other leukocytic cell lines, such as 32D and murine HT-2, which are susceptible to 24p3-mediated apoptosis but not to nonhematopoietic cell lines, such as murine NIH 3T3 and COS-7, which are resistant.	bind
29664	7	7398	7	NULL	NULL	0	NULL	24p3	NULL		does not bind	NULL				NIH 3T3 	NULL	murine			NULL		0	NULL	NULL	NULL	gw60_science_293_5531_829_s_102	11486081	24p3 also bound specifically to IL-3-dependent primary bone marrow cells and to other leukocytic cell lines, such as 32D and murine HT-2, which are susceptible to 24p3-mediated apoptosis but not to nonhematopoietic cell lines, such as murine NIH 3T3 and COS-7, which are resistant.	bind
29665	8	7398	7	NULL	NULL	0	NULL	24p3d	NULL		does not bind	NULL				COS-7 	NULL				NULL		0	NULL	NULL	NULL	gw60_science_293_5531_829_s_102	11486081	24p3 also bound specifically to IL-3-dependent primary bone marrow cells and to other leukocytic cell lines, such as 32D and murine HT-2, which are susceptible to 24p3-mediated apoptosis but not to nonhematopoietic cell lines, such as murine NIH 3T3 and COS-7, which are resistant.	bind
29666	9	7398	7	NULL	NULL	0	NULL	NIH 3T3 	NULL	murine	is resistant to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_science_293_5531_829_s_102	11486081	24p3 also bound specifically to IL-3-dependent primary bone marrow cells and to other leukocytic cell lines, such as 32D and murine HT-2, which are susceptible to 24p3-mediated apoptosis but not to nonhematopoietic cell lines, such as murine NIH 3T3 and COS-7, which are resistant.	bind
29667	10	7398	7	NULL	NULL	0	NULL	COS-7	NULL		is resistant to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_science_293_5531_829_s_102	11486081	24p3 also bound specifically to IL-3-dependent primary bone marrow cells and to other leukocytic cell lines, such as 32D and murine HT-2, which are susceptible to 24p3-mediated apoptosis but not to nonhematopoietic cell lines, such as murine NIH 3T3 and COS-7, which are resistant.	bind
29668	11	7398	7	NULL	NULL	0	NULL	32D	NULL		is a type of	NULL				leukocytic cell line	NULL				NULL		0	NULL	NULL	NULL	gw60_science_293_5531_829_s_102	11486081	24p3 also bound specifically to IL-3-dependent primary bone marrow cells and to other leukocytic cell lines, such as 32D and murine HT-2, which are susceptible to 24p3-mediated apoptosis but not to nonhematopoietic cell lines, such as murine NIH 3T3 and COS-7, which are resistant.	bind
29669	12	7398	7	NULL	NULL	0	NULL	HT-2	NULL	murine	is a type of	NULL				leukocytic cell line	NULL				NULL		0	NULL	NULL	NULL	gw60_science_293_5531_829_s_102	11486081	24p3 also bound specifically to IL-3-dependent primary bone marrow cells and to other leukocytic cell lines, such as 32D and murine HT-2, which are susceptible to 24p3-mediated apoptosis but not to nonhematopoietic cell lines, such as murine NIH 3T3 and COS-7, which are resistant.	bind
29670	13	7398	7	NULL	NULL	0	NULL	NIH 3T3	NULL	murine	is a type of	NULL				 nonhematopoietic cell line	NULL				NULL		0	NULL	NULL	NULL	gw60_science_293_5531_829_s_102	11486081	24p3 also bound specifically to IL-3-dependent primary bone marrow cells and to other leukocytic cell lines, such as 32D and murine HT-2, which are susceptible to 24p3-mediated apoptosis but not to nonhematopoietic cell lines, such as murine NIH 3T3 and COS-7, which are resistant.	bind
29671	14	7398	7	NULL	NULL	0	NULL	 COS-7	NULL		is a type of	NULL				nonhematopoietic cell line	NULL				NULL		0	NULL	NULL	NULL	gw60_science_293_5531_829_s_102	11486081	24p3 also bound specifically to IL-3-dependent primary bone marrow cells and to other leukocytic cell lines, such as 32D and murine HT-2, which are susceptible to 24p3-mediated apoptosis but not to nonhematopoietic cell lines, such as murine NIH 3T3 and COS-7, which are resistant.	bind
54489	15	7398	7	10	NULL	0	NULL	primary bone marrow cells			is dependent on					IL-3					NULL		0	NULL	NULL	NULL	gw60_science_293_5531_829_s_102	11486081	24p3 also bound specifically to IL-3-dependent primary bone marrow cells and to other leukocytic cell lines, such as 32D and murine HT-2, which are susceptible to 24p3-mediated apoptosis but not to nonhematopoietic cell lines, such as murine NIH 3T3 and COS-7, which are resistant.	bind
27449	1	7399	5	13	NULL	NULL	NULL	Smad3	GP		bind		directly			plasminogen activator inhibitor-type 1 gene	GP	human		TGF-beta-inducible elements in promoter	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_515_s_342	11788714	25       Dennler,S., Itoh,S., Vivien,D., ten Dijke,P., Huet,S. and Gauthier,J.-M. (1998) Direct binding of Smad3 and Smad4 to critical TGF-beta-inducible elements in the promoter of human plasminogen activator inhibitor-type 1 gene.	bind
27451	2	7399	5	13	NULL	NULL	NULL	Smad4	GP		bind		directly			plasminogen activator inhibitor-type 1 gene	GP	human		TGF-beta-inducible elements in promoter	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_515_s_342	11788714	25       Dennler,S., Itoh,S., Vivien,D., ten Dijke,P., Huet,S. and Gauthier,J.-M. (1998) Direct binding of Smad3 and Smad4 to critical TGF-beta-inducible elements in the promoter of human plasminogen activator inhibitor-type 1 gene.	bind
29672	1	7399	7	NULL	NULL	0	NULL	Smad3 	NULL		bind	NULL	directly			plasminogen activator inhibitor-type 1 gene	NULL	human		TGF-beta-inducible elements in the promoter of	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_515_s_342	11788714	25       Dennler,S., Itoh,S., Vivien,D., ten Dijke,P., Huet,S. and Gauthier,J.-M. (1998) Direct binding of Smad3 and Smad4 to critical TGF-beta-inducible elements in the promoter of human plasminogen activator inhibitor-type 1 gene.	bind
29673	2	7399	7	NULL	NULL	0	NULL	Smad4	NULL		bind	NULL	directly			plasminogen activator inhibitor-type 1 gene	NULL	human		TGF-beta-inducible elements in the promoter of	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_515_s_342	11788714	25       Dennler,S., Itoh,S., Vivien,D., ten Dijke,P., Huet,S. and Gauthier,J.-M. (1998) Direct binding of Smad3 and Smad4 to critical TGF-beta-inducible elements in the promoter of human plasminogen activator inhibitor-type 1 gene.	bind
27452	1	7400	5	13	NULL	NULL	NULL	p53	GP		bind		sequence-specific			DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_4994_s_321	11812829	25       Gu,W. and Roeder,R.G. (1997) Activation of p53 sequence-specific DNA binding by acetylation of the p53 C-terminal domain.	bind
27453	2	7400	5	13	NULL	NULL	NULL	p53	GP		udergoes			C-terminal domain		acetylation	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_4994_s_321	11812829	25       Gu,W. and Roeder,R.G. (1997) Activation of p53 sequence-specific DNA binding by acetylation of the p53 C-terminal domain.	bind
27454	3	7400	5	13	NULL	NULL	NULL	statement 2	Process		activates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_4994_s_321	11812829	25       Gu,W. and Roeder,R.G. (1997) Activation of p53 sequence-specific DNA binding by acetylation of the p53 C-terminal domain.	bind
29674	1	7400	7	10	NULL	0	NULL	p53			undergoes			C-terminal domain		acetylation					NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_4994_s_321	11812829	25       Gu,W. and Roeder,R.G. (1997) Activation of p53 sequence-specific DNA binding by acetylation of the p53 C-terminal domain.	bind
29675	2	7400	7	10	NULL	0	NULL	statement 1			activates					statement 3					NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_4994_s_321	11812829	25       Gu,W. and Roeder,R.G. (1997) Activation of p53 sequence-specific DNA binding by acetylation of the p53 C-terminal domain.	bind
54490	3	7400	7	10	NULL	0	NULL	p53			bind		sequence specifically			DNA					NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_4994_s_321	11812829	25       Gu,W. and Roeder,R.G. (1997) Activation of p53 sequence-specific DNA binding by acetylation of the p53 C-terminal domain.	bind
27455	1	7401	5	13	NULL	NULL	NULL	nuclear proteins	GP		bind					pre-mRNA	NucleicAcid			r(UUAG/G)	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_11_2268_s_334	11376145	25       Ishikawa,F., Matunis,M.J., Dreyfuss,G. and Cech,T.R. (1993) Nuclear proteins that bind the pre-mRNA 3' splice site sequence r(UUAG/G) and the human telomeric DNA sequence d(TTAGGG)n.  Mol.	bind
27456	2	7401	5	13	NULL	NULL	NULL	r(UUAG/G)	NucleicAcid		is a type of					3' splice site sequence	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_11_2268_s_334	11376145	25       Ishikawa,F., Matunis,M.J., Dreyfuss,G. and Cech,T.R. (1993) Nuclear proteins that bind the pre-mRNA 3' splice site sequence r(UUAG/G) and the human telomeric DNA sequence d(TTAGGG)n.  Mol.	bind
27457	3	7401	5	13	NULL	NULL	NULL	nuclear proteins	GP		bind							human		d(TTAGGG)n	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_11_2268_s_334	11376145	25       Ishikawa,F., Matunis,M.J., Dreyfuss,G. and Cech,T.R. (1993) Nuclear proteins that bind the pre-mRNA 3' splice site sequence r(UUAG/G) and the human telomeric DNA sequence d(TTAGGG)n.  Mol.	bind
27458	4	7401	5	13	NULL	NULL	NULL	d(TTAGGG)n	NucleicAcid		is a type of					telomeric DNA sequence	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_11_2268_s_334	11376145	25       Ishikawa,F., Matunis,M.J., Dreyfuss,G. and Cech,T.R. (1993) Nuclear proteins that bind the pre-mRNA 3' splice site sequence r(UUAG/G) and the human telomeric DNA sequence d(TTAGGG)n.  Mol.	bind
29676	1	7401	7	10	NULL	0	NULL	Nuclear proteins			bind					pre-mRNA			r(UUAG/G)		NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_11_2268_s_334	11376145	25       Ishikawa,F., Matunis,M.J., Dreyfuss,G. and Cech,T.R. (1993) Nuclear proteins that bind the pre-mRNA 3' splice site sequence r(UUAG/G) and the human telomeric DNA sequence d(TTAGGG)n.  Mol.	bind
29677	2	7401	7	10	NULL	0	NULL	Nuclear proteins 			bind							human		d(TTAGGG)	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_11_2268_s_334	11376145	25       Ishikawa,F., Matunis,M.J., Dreyfuss,G. and Cech,T.R. (1993) Nuclear proteins that bind the pre-mRNA 3' splice site sequence r(UUAG/G) and the human telomeric DNA sequence d(TTAGGG)n.  Mol.	bind
54499	3	7401	7	10	NULL	0	NULL	d(TTAGGG)n			is a type of					telomeric DNA sequence					NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_11_2268_s_334	11376145	25       Ishikawa,F., Matunis,M.J., Dreyfuss,G. and Cech,T.R. (1993) Nuclear proteins that bind the pre-mRNA 3' splice site sequence r(UUAG/G) and the human telomeric DNA sequence d(TTAGGG)n.  Mol.	bind
54500	5	7401	7	10	NULL	0	NULL	r(UUAG/G)			is a type of					3' splice site sequence					NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_11_2268_s_334	11376145	25       Ishikawa,F., Matunis,M.J., Dreyfuss,G. and Cech,T.R. (1993) Nuclear proteins that bind the pre-mRNA 3' splice site sequence r(UUAG/G) and the human telomeric DNA sequence d(TTAGGG)n.  Mol.	bind
27463	1	7404	5	13	NULL	NULL	NULL	Rb	GP	active	bind					E2Fs	GP				NULL	repressor complex	NULL	NULL	NULL	NULL	gw60_amjpathol_157_6_1795_s_155	11106551	25  Active Rb is normally bound to E2Fs in a repressor complex.	bind
29679	1	7404	7	NULL	NULL	0	NULL	Rb	NULL	active	bind	NULL				E2Fs	NULL				NULL	repressor complex	0	NULL	NULL	NULL	gw60_amjpathol_157_6_1795_s_155	11106551	25  Active Rb is normally bound to E2Fs in a repressor complex.	bind
27698	1	7405	5	NULL	NULL	0	NULL		NULL		stabilizes	NULL		Arginine 3500			NULL	clusters of amino acids	3147 to 3157		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_10_1719_s_153	7583549	25  Arginine 3500 is suggested to stabilize two clusters of amino acids (3147 to 3157 and 3359 to 3367) that have been assumed to ensure the binding of the apoB to the LDL receptor.	bind
27699	2	7405	5	NULL	NULL	0	NULL		NULL		stabilizes	NULL		Arginine 3500			NULL	clusters of amino acids	3359 to 3367		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_10_1719_s_153	7583549	25  Arginine 3500 is suggested to stabilize two clusters of amino acids (3147 to 3157 and 3359 to 3367) that have been assumed to ensure the binding of the apoB to the LDL receptor.	bind
27700	3	7405	5	13	NULL	NULL	NULL	apoB	GP		bind					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_10_1719_s_153	7583549	25  Arginine 3500 is suggested to stabilize two clusters of amino acids (3147 to 3157 and 3359 to 3367) that have been assumed to ensure the binding of the apoB to the LDL receptor.	bind
27701	4	7405	5	13	NULL	NULL	NULL	statement 1	Process		ensure					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_10_1719_s_153	7583549	25  Arginine 3500 is suggested to stabilize two clusters of amino acids (3147 to 3157 and 3359 to 3367) that have been assumed to ensure the binding of the apoB to the LDL receptor.	bind
27702	5	7405	5	13	NULL	NULL	NULL	statement 2	Process		ensure					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_10_1719_s_153	7583549	25  Arginine 3500 is suggested to stabilize two clusters of amino acids (3147 to 3157 and 3359 to 3367) that have been assumed to ensure the binding of the apoB to the LDL receptor.	bind
29680	1	7405	7	NULL	NULL	0	NULL	apoB	NULL		bind	NULL				LDL receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_10_1719_s_153	7583549	25  Arginine 3500 is suggested to stabilize two clusters of amino acids (3147 to 3157 and 3359 to 3367) that have been assumed to ensure the binding of the apoB to the LDL receptor.	bind
29681	2	7405	7	NULL	NULL	0	NULL		NULL		stabilize	NULL		Arginine 3500			NULL		aminoacids 3147 to 3157		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_10_1719_s_153	7583549	25  Arginine 3500 is suggested to stabilize two clusters of amino acids (3147 to 3157 and 3359 to 3367) that have been assumed to ensure the binding of the apoB to the LDL receptor.	bind
29682	3	7405	7	NULL	NULL	0	NULL		NULL		stabilize	NULL		Arginine 3500			NULL		aminoacids 3359 to 3367		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_10_1719_s_153	7583549	25  Arginine 3500 is suggested to stabilize two clusters of amino acids (3147 to 3157 and 3359 to 3367) that have been assumed to ensure the binding of the apoB to the LDL receptor.	bind
29683	4	7405	7	NULL	NULL	0	NULL	statement 2	NULL		ensures	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_10_1719_s_153	7583549	25  Arginine 3500 is suggested to stabilize two clusters of amino acids (3147 to 3157 and 3359 to 3367) that have been assumed to ensure the binding of the apoB to the LDL receptor.	bind
29684	5	7405	7	NULL	NULL	0	NULL	statement 3	NULL		ensures	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_10_1719_s_153	7583549	25  Arginine 3500 is suggested to stabilize two clusters of amino acids (3147 to 3157 and 3359 to 3367) that have been assumed to ensure the binding of the apoB to the LDL receptor.	bind
27703	1	7406	5	13	NULL	NULL	NULL	ADP	Chemical		bind					CMK 11-5 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_190	9108793	25  In addition, neither GDP nor adenosine competed significantly with the binding of ADP to CMK 11-5 cells, indicating the absence of other purinergic receptors.	bind
27704	2	7406	5	13	NULL	NULL	NULL	GDP	Chemical		does not compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_190	9108793	25  In addition, neither GDP nor adenosine competed significantly with the binding of ADP to CMK 11-5 cells, indicating the absence of other purinergic receptors.	bind
27705	3	7406	5	13	NULL	NULL	NULL	adenosine	Chemical		does not compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_190	9108793	25  In addition, neither GDP nor adenosine competed significantly with the binding of ADP to CMK 11-5 cells, indicating the absence of other purinergic receptors.	bind
27706	4	7406	5	13	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_190	9108793	25  In addition, neither GDP nor adenosine competed significantly with the binding of ADP to CMK 11-5 cells, indicating the absence of other purinergic receptors.	bind
27707	5	7406	5	13	NULL	NULL	NULL	statement 2	Process		indicates					purinergic receptors	GP	absence of other			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_190	9108793	25  In addition, neither GDP nor adenosine competed significantly with the binding of ADP to CMK 11-5 cells, indicating the absence of other purinergic receptors.	bind
27708	6	7406	5	13	NULL	NULL	NULL	statement 3	Process		indicates					purinergic receptors	GP	absence of other			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_190	9108793	25  In addition, neither GDP nor adenosine competed significantly with the binding of ADP to CMK 11-5 cells, indicating the absence of other purinergic receptors.	bind
29685	1	7406	7	NULL	NULL	0	NULL	ADP	NULL		binds	NULL				CMK 11-5 cells	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_190	9108793	25  In addition, neither GDP nor adenosine competed significantly with the binding of ADP to CMK 11-5 cells, indicating the absence of other purinergic receptors.	bind
29686	2	7406	7	NULL	NULL	0	NULL	GDP	NULL		does not compete with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_190	9108793	25  In addition, neither GDP nor adenosine competed significantly with the binding of ADP to CMK 11-5 cells, indicating the absence of other purinergic receptors.	bind
29687	3	7406	7	NULL	NULL	0	NULL	adenosine	NULL		does not compete with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_190	9108793	25  In addition, neither GDP nor adenosine competed significantly with the binding of ADP to CMK 11-5 cells, indicating the absence of other purinergic receptors.	bind
29688	4	7406	7	NULL	NULL	0	NULL	statement 2	NULL		indicate	NULL				purinergic receptors	NULL	absence of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_190	9108793	25  In addition, neither GDP nor adenosine competed significantly with the binding of ADP to CMK 11-5 cells, indicating the absence of other purinergic receptors.	bind
29689	5	7406	7	NULL	NULL	0	NULL	statement 3	NULL		indicate	NULL				purinergic receptors	NULL	absence of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_190	9108793	25  In addition, neither GDP nor adenosine competed significantly with the binding of ADP to CMK 11-5 cells, indicating the absence of other purinergic receptors.	bind
27709	1	7407	5	13	NULL	NULL	NULL	PAF-acetylhydrolase	GP		inactivates					PAF	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_4_787_s_61	9054729	25  PAF is inactivated by PAF-acetylhydrolase, an enzyme that circulates bound to LDL.	bind
27710	2	7407	5	13	NULL	NULL	NULL	PAF-acetylhydrolase	GP		bind					LDL	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_4_787_s_61	9054729	25  PAF is inactivated by PAF-acetylhydrolase, an enzyme that circulates bound to LDL.	bind
29690	1	7407	7	NULL	NULL	0	NULL	PAF-acetylhydrolase	NULL		inactivates	NULL				PAF	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_95_4_787_s_61	9054729	25  PAF is inactivated by PAF-acetylhydrolase, an enzyme that circulates bound to LDL.	bind
29691	2	7407	7	NULL	NULL	0	NULL	PAF-acetylhydrolase	NULL		bind	NULL				LDL	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_95_4_787_s_61	9054729	25  PAF is inactivated by PAF-acetylhydrolase, an enzyme that circulates bound to LDL.	bind
29692	3	7407	7	NULL	NULL	0	NULL	PAF-acetylhydrolase	NULL		is a type of	NULL				enzyme	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_95_4_787_s_61	9054729	25  PAF is inactivated by PAF-acetylhydrolase, an enzyme that circulates bound to LDL.	bind
27711	1	7408	5	13	NULL	NULL	NULL	apoB-100	GP		is a component of					LDL	GP	granule-bound			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_11_2047_s_145	7583588	25  When the apoB-100 component of granule-bound LDL is proteolyzed by granule chymase, the LDL particles become unstable and fuse, and the fused particles bind more tightly to the granule remnant heparin proteoglycans.	bind
27712	2	7408	5	13	NULL	NULL	NULL	statement 1	GP		is proteolyzed by					granule chymase	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_11_2047_s_145	7583588	25  When the apoB-100 component of granule-bound LDL is proteolyzed by granule chymase, the LDL particles become unstable and fuse, and the fused particles bind more tightly to the granule remnant heparin proteoglycans.	bind
27713	3	7408	5	13	NULL	NULL	NULL	statement 2	Process		leads to					LDL particles	GP	unstable			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_11_2047_s_145	7583588	25  When the apoB-100 component of granule-bound LDL is proteolyzed by granule chymase, the LDL particles become unstable and fuse, and the fused particles bind more tightly to the granule remnant heparin proteoglycans.	bind
27714	4	7408	5	13	NULL	NULL	NULL	statement 3	Process		results in					LDL particles	GP	fusion of;;unstable			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_11_2047_s_145	7583588	25  When the apoB-100 component of granule-bound LDL is proteolyzed by granule chymase, the LDL particles become unstable and fuse, and the fused particles bind more tightly to the granule remnant heparin proteoglycans.	bind
27715	5	7408	5	13	NULL	NULL	NULL	LDL particles	GP	fused	bind		tightly			heparin proteoglycans	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_11_2047_s_145	7583588	25  When the apoB-100 component of granule-bound LDL is proteolyzed by granule chymase, the LDL particles become unstable and fuse, and the fused particles bind more tightly to the granule remnant heparin proteoglycans.	bind
54501	6	7408	5	13	NULL	NULL	NULL	heparin proteoglycans \t	GP		is a type of					granule remnant	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_11_2047_s_145	7583588	25  When the apoB-100 component of granule-bound LDL is proteolyzed by granule chymase, the LDL particles become unstable and fuse, and the fused particles bind more tightly to the granule remnant heparin proteoglycans.	bind
29706	1	7408	7	NULL	NULL	0	NULL	granule	NULL	apoB-100	bind	NULL				LDL	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_11_2047_s_145	7583588	25  When the apoB-100 component of granule-bound LDL is proteolyzed by granule chymase, the LDL particles become unstable and fuse, and the fused particles bind more tightly to the granule remnant heparin proteoglycans.	bind
29707	2	7408	7	NULL	NULL	0	NULL	granule chymase	NULL		proteolyze	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_11_2047_s_145	7583588	25  When the apoB-100 component of granule-bound LDL is proteolyzed by granule chymase, the LDL particles become unstable and fuse, and the fused particles bind more tightly to the granule remnant heparin proteoglycans.	bind
29710	3	7408	7	NULL	NULL	0	NULL	LDL particles	NULL		become	NULL				unstable	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_11_2047_s_145	7583588	25  When the apoB-100 component of granule-bound LDL is proteolyzed by granule chymase, the LDL particles become unstable and fuse, and the fused particles bind more tightly to the granule remnant heparin proteoglycans.	bind
29712	4	7408	7	NULL	NULL	0	NULL	statement 3	NULL		leads to	NULL				LDL particles	NULL	fusion of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_11_2047_s_145	7583588	25  When the apoB-100 component of granule-bound LDL is proteolyzed by granule chymase, the LDL particles become unstable and fuse, and the fused particles bind more tightly to the granule remnant heparin proteoglycans.	bind
29713	5	7408	7	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_11_2047_s_145	7583588	25  When the apoB-100 component of granule-bound LDL is proteolyzed by granule chymase, the LDL particles become unstable and fuse, and the fused particles bind more tightly to the granule remnant heparin proteoglycans.	bind
29715	6	7408	7	NULL	NULL	0	NULL	LDL	NULL	fused particles	bind	NULL	tightly			heparin proteoglycans	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_11_2047_s_145	7583588	25  When the apoB-100 component of granule-bound LDL is proteolyzed by granule chymase, the LDL particles become unstable and fuse, and the fused particles bind more tightly to the granule remnant heparin proteoglycans.	bind
29716	7	7408	7	NULL	NULL	0	NULL	heparin proteoglycans	NULL		is a type of	NULL				granule remnant	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_11_2047_s_145	7583588	25  When the apoB-100 component of granule-bound LDL is proteolyzed by granule chymase, the LDL particles become unstable and fuse, and the fused particles bind more tightly to the granule remnant heparin proteoglycans.	bind
27716	1	7409	5	13	NULL	NULL	NULL	uPAR	GP	recombinant	bind					vitronectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_12_1855_s_41	9848876	25 26  Recombinant uPAR binds vitronectin, and this binding is augmented by the addition of uPA.	bind
27717	2	7409	5	13	NULL	NULL	NULL	uPA	GP		augments					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_12_1855_s_41	9848876	25 26  Recombinant uPAR binds vitronectin, and this binding is augmented by the addition of uPA.	bind
29854	1	7409	7	NULL	NULL	0	NULL	uPAR	NULL	recombinant	binds	NULL				vitronectin	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_12_1855_s_41	9848876	25 26  Recombinant uPAR binds vitronectin, and this binding is augmented by the addition of uPA.	bind
29855	2	7409	7	NULL	NULL	0	NULL	uPA	NULL		augments	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_12_1855_s_41	9848876	25 26  Recombinant uPAR binds vitronectin, and this binding is augmented by the addition of uPA.	bind
29604	1	7410	5	13	NULL	NULL	NULL	Glanzmann's thrombasthenic platelets	Cell		lack					GP IIb/IIa	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_34	9108793	25 26 27  Glanzmann's thrombasthenic platelets, despite the absence of GP IIb/IIa, show binding of ADP and ATP-alpha-S similar to that of control platelets, normal ADP-induced Ca2+ influx, platelet shape change, and inhibition of cAMP levels, 28 29 30  although their ability to synthesize thromboxane B2 is reduced.	bind
29605	2	7410	5	13	NULL	NULL	NULL	statement 1	Cell		bind					ADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_34	9108793	25 26 27  Glanzmann's thrombasthenic platelets, despite the absence of GP IIb/IIa, show binding of ADP and ATP-alpha-S similar to that of control platelets, normal ADP-induced Ca2+ influx, platelet shape change, and inhibition of cAMP levels, 28 29 30  although their ability to synthesize thromboxane B2 is reduced.	bind
29606	3	7410	5	13	NULL	NULL	NULL	statement 1	Cell		bind					ATP-alpha-S	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_34	9108793	25 26 27  Glanzmann's thrombasthenic platelets, despite the absence of GP IIb/IIa, show binding of ADP and ATP-alpha-S similar to that of control platelets, normal ADP-induced Ca2+ influx, platelet shape change, and inhibition of cAMP levels, 28 29 30  although their ability to synthesize thromboxane B2 is reduced.	bind
29607	4	7410	5	13	NULL	NULL	NULL	ADP	Chemical		induces					Ca2+ influx	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_34	9108793	25 26 27  Glanzmann's thrombasthenic platelets, despite the absence of GP IIb/IIa, show binding of ADP and ATP-alpha-S similar to that of control platelets, normal ADP-induced Ca2+ influx, platelet shape change, and inhibition of cAMP levels, 28 29 30  although their ability to synthesize thromboxane B2 is reduced.	bind
29608	5	7410	5	13	NULL	NULL	NULL	statement 4	Process		occurs in					statement 1	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_34	9108793	25 26 27  Glanzmann's thrombasthenic platelets, despite the absence of GP IIb/IIa, show binding of ADP and ATP-alpha-S similar to that of control platelets, normal ADP-induced Ca2+ influx, platelet shape change, and inhibition of cAMP levels, 28 29 30  although their ability to synthesize thromboxane B2 is reduced.	bind
29609	6	7410	5	13	NULL	NULL	NULL	platelet	Cell	shape change in	occurs in					statement 1	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_34	9108793	25 26 27  Glanzmann's thrombasthenic platelets, despite the absence of GP IIb/IIa, show binding of ADP and ATP-alpha-S similar to that of control platelets, normal ADP-induced Ca2+ influx, platelet shape change, and inhibition of cAMP levels, 28 29 30  although their ability to synthesize thromboxane B2 is reduced.	bind
29610	7	7410	5	13	NULL	NULL	NULL	cAMP	Chemical	inhibition of	occurs in					statement 1	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_34	9108793	25 26 27  Glanzmann's thrombasthenic platelets, despite the absence of GP IIb/IIa, show binding of ADP and ATP-alpha-S similar to that of control platelets, normal ADP-induced Ca2+ influx, platelet shape change, and inhibition of cAMP levels, 28 29 30  although their ability to synthesize thromboxane B2 is reduced.	bind
29611	8	7410	5	13	NULL	NULL	NULL	thromboxane B2	Chemical	ability to synthesize	is reduced in					statement 1	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_34	9108793	25 26 27  Glanzmann's thrombasthenic platelets, despite the absence of GP IIb/IIa, show binding of ADP and ATP-alpha-S similar to that of control platelets, normal ADP-induced Ca2+ influx, platelet shape change, and inhibition of cAMP levels, 28 29 30  although their ability to synthesize thromboxane B2 is reduced.	bind
29856	1	7410	7	10	NULL	0	NULL	Glanzmann's thrombasthenic platelets	NULL		bind	NULL				ADP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_34	9108793	25 26 27  Glanzmann's thrombasthenic platelets, despite the absence of GP IIb/IIa, show binding of ADP and ATP-alpha-S similar to that of control platelets, normal ADP-induced Ca2+ influx, platelet shape change, and inhibition of cAMP levels, 28 29 30  although their ability to synthesize thromboxane B2 is reduced.	bind
29857	2	7410	7	10	NULL	0	NULL	Glanzmann's thrombasthenic platelets	NULL		bind	NULL				ATP-alpha-S	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_34	9108793	25 26 27  Glanzmann's thrombasthenic platelets, despite the absence of GP IIb/IIa, show binding of ADP and ATP-alpha-S similar to that of control platelets, normal ADP-induced Ca2+ influx, platelet shape change, and inhibition of cAMP levels, 28 29 30  although their ability to synthesize thromboxane B2 is reduced.	bind
29858	3	7410	7	NULL	NULL	0	NULL	statement 1	NULL		in absence of	NULL				GP IIb/IIa	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_34	9108793	25 26 27  Glanzmann's thrombasthenic platelets, despite the absence of GP IIb/IIa, show binding of ADP and ATP-alpha-S similar to that of control platelets, normal ADP-induced Ca2+ influx, platelet shape change, and inhibition of cAMP levels, 28 29 30  although their ability to synthesize thromboxane B2 is reduced.	bind
29859	4	7410	7	NULL	NULL	0	NULL	statement 2	NULL		in absence of	NULL				GP IIb/IIa	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_34	9108793	25 26 27  Glanzmann's thrombasthenic platelets, despite the absence of GP IIb/IIa, show binding of ADP and ATP-alpha-S similar to that of control platelets, normal ADP-induced Ca2+ influx, platelet shape change, and inhibition of cAMP levels, 28 29 30  although their ability to synthesize thromboxane B2 is reduced.	bind
29860	5	7410	7	NULL	NULL	0	NULL	ADP	NULL	normal	induce	NULL				Ca2+	NULL	influx of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_34	9108793	25 26 27  Glanzmann's thrombasthenic platelets, despite the absence of GP IIb/IIa, show binding of ADP and ATP-alpha-S similar to that of control platelets, normal ADP-induced Ca2+ influx, platelet shape change, and inhibition of cAMP levels, 28 29 30  although their ability to synthesize thromboxane B2 is reduced.	bind
29861	6	7410	7	NULL	NULL	0	NULL	ADP	NULL	normal	change	NULL				platelet shape	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_34	9108793	25 26 27  Glanzmann's thrombasthenic platelets, despite the absence of GP IIb/IIa, show binding of ADP and ATP-alpha-S similar to that of control platelets, normal ADP-induced Ca2+ influx, platelet shape change, and inhibition of cAMP levels, 28 29 30  although their ability to synthesize thromboxane B2 is reduced.	bind
29862	7	7410	7	NULL	NULL	0	NULL	ADP	NULL	normal	inhibits	NULL				cAMP	NULL	levels of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_34	9108793	25 26 27  Glanzmann's thrombasthenic platelets, despite the absence of GP IIb/IIa, show binding of ADP and ATP-alpha-S similar to that of control platelets, normal ADP-induced Ca2+ influx, platelet shape change, and inhibition of cAMP levels, 28 29 30  although their ability to synthesize thromboxane B2 is reduced.	bind
29863	8	7410	7	NULL	NULL	0	NULL	platelets	NULL	control	bind	NULL				ADP	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_34	9108793	25 26 27  Glanzmann's thrombasthenic platelets, despite the absence of GP IIb/IIa, show binding of ADP and ATP-alpha-S similar to that of control platelets, normal ADP-induced Ca2+ influx, platelet shape change, and inhibition of cAMP levels, 28 29 30  although their ability to synthesize thromboxane B2 is reduced.	bind
29864	9	7410	7	NULL	NULL	0	NULL	platelets	NULL	normal	bind	NULL				ATP-alpha-S	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_34	9108793	25 26 27  Glanzmann's thrombasthenic platelets, despite the absence of GP IIb/IIa, show binding of ADP and ATP-alpha-S similar to that of control platelets, normal ADP-induced Ca2+ influx, platelet shape change, and inhibition of cAMP levels, 28 29 30  although their ability to synthesize thromboxane B2 is reduced.	bind
29866	10	7410	7	NULL	NULL	0	NULL	statement 1	NULL		is similar to	NULL				statement 8	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_34	9108793	25 26 27  Glanzmann's thrombasthenic platelets, despite the absence of GP IIb/IIa, show binding of ADP and ATP-alpha-S similar to that of control platelets, normal ADP-induced Ca2+ influx, platelet shape change, and inhibition of cAMP levels, 28 29 30  although their ability to synthesize thromboxane B2 is reduced.	bind
29867	11	7410	7	NULL	NULL	0	NULL	statement 2	NULL		is similar to	NULL				statement 9	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_34	9108793	25 26 27  Glanzmann's thrombasthenic platelets, despite the absence of GP IIb/IIa, show binding of ADP and ATP-alpha-S similar to that of control platelets, normal ADP-induced Ca2+ influx, platelet shape change, and inhibition of cAMP levels, 28 29 30  although their ability to synthesize thromboxane B2 is reduced.	bind
29868	12	7410	7	NULL	NULL	0	NULL	ADP	NULL	normal	reduce	NULL				thromboxane B2	NULL	synthesis of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_4_769_s_34	9108793	25 26 27  Glanzmann's thrombasthenic platelets, despite the absence of GP IIb/IIa, show binding of ADP and ATP-alpha-S similar to that of control platelets, normal ADP-induced Ca2+ influx, platelet shape change, and inhibition of cAMP levels, 28 29 30  although their ability to synthesize thromboxane B2 is reduced.	bind
27718	1	7411	5	13	NULL	NULL	NULL	IRF-1	GP	competitive binding of	plays a role in		critical			growth	Process	determining			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_2_233_s_173	10666420	25 26 27 47 48 49 50  Recently, competitive binding of IRF-1 and IRF-2 was reported to play a critical role in determining growth, transformation, and apoptosis of cells.	bind
27719	2	7411	5	13	NULL	NULL	NULL	IRF-2	GP	competitive binding of	plays a role in		critical			growth	Process	determining			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_2_233_s_173	10666420	25 26 27 47 48 49 50  Recently, competitive binding of IRF-1 and IRF-2 was reported to play a critical role in determining growth, transformation, and apoptosis of cells.	bind
27720	3	7411	5	13	NULL	NULL	NULL	IRF-1	GP	competitive binding of	plays a role in		critical			transformation	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_2_233_s_173	10666420	25 26 27 47 48 49 50  Recently, competitive binding of IRF-1 and IRF-2 was reported to play a critical role in determining growth, transformation, and apoptosis of cells.	bind
27721	4	7411	5	13	NULL	NULL	NULL	IRF-2	GP	competitive binding of	plays a role in		critical			transformation	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_2_233_s_173	10666420	25 26 27 47 48 49 50  Recently, competitive binding of IRF-1 and IRF-2 was reported to play a critical role in determining growth, transformation, and apoptosis of cells.	bind
27722	5	7411	5	13	NULL	NULL	NULL	IRF-1	GP	competitive binding of	plays a role in		critical			apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_2_233_s_173	10666420	25 26 27 47 48 49 50  Recently, competitive binding of IRF-1 and IRF-2 was reported to play a critical role in determining growth, transformation, and apoptosis of cells.	bind
27723	6	7411	5	13	NULL	NULL	NULL	IRF-2	GP	competitive binding of	plays a role in		critical			apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_2_233_s_173	10666420	25 26 27 47 48 49 50  Recently, competitive binding of IRF-1 and IRF-2 was reported to play a critical role in determining growth, transformation, and apoptosis of cells.	bind
29871	1	7411	7	10	NULL	0	NULL	IRF-1	NULL	competitive binding of	plays a role in	NULL	critical			growth	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_2_233_s_173	10666420	25 26 27 47 48 49 50  Recently, competitive binding of IRF-1 and IRF-2 was reported to play a critical role in determining growth, transformation, and apoptosis of cells.	bind
29873	2	7411	7	10	NULL	0	NULL	IRF-1	NULL	competitive binding of	plays a role in	NULL	critical			transformation	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_2_233_s_173	10666420	25 26 27 47 48 49 50  Recently, competitive binding of IRF-1 and IRF-2 was reported to play a critical role in determining growth, transformation, and apoptosis of cells.	bind
29875	3	7411	7	10	NULL	0	NULL	IRF-1	NULL	competitive binding of	plays a role in	NULL	critical			apoptosis of cells	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_2_233_s_173	10666420	25 26 27 47 48 49 50  Recently, competitive binding of IRF-1 and IRF-2 was reported to play a critical role in determining growth, transformation, and apoptosis of cells.	bind
29877	4	7411	7	10	NULL	0	NULL	IRF-2	NULL	competitive binding of	plays a role in	NULL	critical			growth	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_2_233_s_173	10666420	25 26 27 47 48 49 50  Recently, competitive binding of IRF-1 and IRF-2 was reported to play a critical role in determining growth, transformation, and apoptosis of cells.	bind
29878	5	7411	7	10	NULL	0	NULL	IRF-2	NULL	competitive binding of	plays a role in	NULL	critical			transformation	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_2_233_s_173	10666420	25 26 27 47 48 49 50  Recently, competitive binding of IRF-1 and IRF-2 was reported to play a critical role in determining growth, transformation, and apoptosis of cells.	bind
29879	6	7411	7	10	NULL	0	NULL	IRF-2	NULL	competitive binding of	plays a role in	NULL	critical			apoptosis of cells	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_2_233_s_173	10666420	25 26 27 47 48 49 50  Recently, competitive binding of IRF-1 and IRF-2 was reported to play a critical role in determining growth, transformation, and apoptosis of cells.	bind
27724	1	7412	5	13	NULL	NULL	NULL	Lp(a)	GP		bind		weakly			LDLR	GP				NULL	yolk sac cell line 1461	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_552_s_262	10073957	25 62 63 However, because the yolk sac cell line 1461 was shown to express slightly higher amounts of LDLR than did control cells (Figure 1B  ), it was essential to make sure that the weak Lp(a) binding to the LDLR was of negligible influence within the assay system used in this study.	bind
29884	1	7412	7	10	NULL	0	NULL	Lp(a)	NULL		bind	NULL	weakly			LDLR	NULL				NULL	 yolk sac cell line 1461	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_552_s_262	10073957	25 62 63 However, because the yolk sac cell line 1461 was shown to express slightly higher amounts of LDLR than did control cells (Figure 1B  ), it was essential to make sure that the weak Lp(a) binding to the LDLR was of negligible influence within the assay system used in this study.	bind
27728	1	7413	5	13	NULL	NULL	NULL	ANP	GP		bind					NPR-A receptors	GP				NULL	on adipocytes	NULL	NULL	NULL	NULL	gw70_circulation_109_5_594_s_131	14769680	25 Investigators have demonstrated that binding of ANP to NPR-A receptors on adipocytes induces lipolysis.	bind
27729	2	7413	5	13	NULL	NULL	NULL	statement 1	Process		induces					lipolysis	Process				NULL	adipocytes	NULL	NULL	NULL	NULL	gw70_circulation_109_5_594_s_131	14769680	25 Investigators have demonstrated that binding of ANP to NPR-A receptors on adipocytes induces lipolysis.	bind
29888	1	7413	7	NULL	NULL	0	NULL	ANP	NULL		bind	NULL				NPR-A receptors	NULL				NULL	adipocytes	0	NULL	NULL	NULL	gw70_circulation_109_5_594_s_131	14769680	25 Investigators have demonstrated that binding of ANP to NPR-A receptors on adipocytes induces lipolysis.	bind
29891	2	7413	7	10	NULL	0	NULL	statement 1			induces					lipolysis					NULL	adipocytes	NULL	NULL	NULL	NULL	gw70_circulation_109_5_594_s_131	14769680	25 Investigators have demonstrated that binding of ANP to NPR-A receptors on adipocytes induces lipolysis.	bind
29009	1	7414	5	13	NULL	NULL	NULL	external signals	Process		is linked to					nuclear responses	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29010	2	7414	5	13	NULL	NULL	NULL	MAPKs	GP		is required for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29011	3	7414	5	13	NULL	NULL	NULL	growth factor	GP		bind					RTK	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29012	4	7414	5	13	NULL	NULL	NULL	growth factor	GP		bind					GPCR	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29013	5	7414	5	13	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29014	6	7414	5	13	NULL	NULL	NULL	statement 3	Process		leads to					gene	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29015	7	7414	5	13	NULL	NULL	NULL	MAPKs	GP		is required for					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29016	8	7414	5	13	NULL	NULL	NULL	statement 4	Process		leads to					gene	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29017	9	7414	5	13	NULL	NULL	NULL	MAPKs	GP		is required for					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29515	10	7414	5	13	NULL	NULL	NULL	GPCRs	GP		is coupled to					Galphaq	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29516	11	7414	5	13	NULL	NULL	NULL	GPCRs	GP		is coupled to					Galphai	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29517	12	7414	5	13	NULL	NULL	NULL	statement 10	Process	activation of	triggers					Ras	GP	action of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29518	13	7414	5	13	NULL	NULL	NULL	statement 12	Process		occurs during					MAPK signal transduction	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
30123	14	7414	5	13	NULL	NULL	NULL	statement 11	Process	activation of	triggers					Ras	GP	action of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
30124	15	7414	5	13	NULL	NULL	NULL	statement 14	Process		occurs during					MAPK signal transduction	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
30125	16	7414	5	13	NULL	NULL	NULL	GPCRs	GP	stimulation of	induces		rapidly			Shc	GP	phosphorylation of	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
30126	17	7414	5	13	NULL	NULL	NULL	Shc	GP		bind					Grb2	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
30127	18	7414	5	13	NULL	NULL	NULL	GPCRs	GP	stimulation of	induces		rapidly			statement 17	Process	formation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
30128	19	7414	5	13	NULL	NULL	NULL	GPCR	GP		is coupled to					Ras	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
30129	20	7414	5	13	NULL	NULL	NULL	RTK	GP		is coupled to					Ras	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
30130	21	7414	5	13	NULL	NULL	NULL	statement 16	Process		is required for					statement 19	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
30131	22	7414	5	13	NULL	NULL	NULL	statement 16	Process		is required for					statement 20	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
30132	23	7414	5	13	NULL	NULL	NULL	statement 18	Process		is required for					statement 19	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
30133	24	7414	5	13	NULL	NULL	NULL	statement 18	Process		is required for					statement 20	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
30134	25	7414	5	13	NULL	NULL	NULL	lysophosphatidic acid receptor	GP		is a type of					GPCRs	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
30135	26	7414	5	13	NULL	NULL	NULL	thyroid-releasing hormone receptor	GP		is a type of					GPCRs	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
30136	27	7414	5	13	NULL	NULL	NULL	endothelin-1 receptor	GP		is a type of					GPCRs	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
30137	28	7414	5	13	NULL	NULL	NULL	bradykinin receptor	GP		is a type of					GPCRs	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29893	1	7414	7	NULL	NULL	0	NULL	growth factor	NULL		bind	NULL				RTK	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29894	2	7414	7	NULL	NULL	0	NULL	growth factor	NULL		bind	NULL				GPCR	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29895	3	7414	7	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29896	4	7414	7	NULL	NULL	0	NULL	MAPKs	NULL		link	NULL				gene expression	NULL	external signals to			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29898	5	7414	7	NULL	NULL	0	NULL	statement 4	NULL		in response to	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29899	6	7414	7	NULL	NULL	0	NULL	statement 4	NULL		in response to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29901	7	7414	7	10	NULL	0	NULL	Galphaq		activation of	triggers					Ras		action of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29902	8	7414	7	10	NULL	0	NULL	Galphai-coupled GPCRs		activation of	triggers					Ras		action of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29905	9	7414	7	NULL	NULL	0	NULL	lysophosphatidic acid receptor	NULL		induce	NULL	rapidly			Shc	NULL	phosphorylation of	tyrosine		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29906	10	7414	7	NULL	NULL	0	NULL	thyroid-releasing hormone receptor	NULL		induce	NULL	rapidly			Shc	NULL	phosphorylation of	tyrosine		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29907	11	7414	7	NULL	NULL	0	NULL	endothelin-1 receptor	NULL		induce	NULL	rapidly			Shc	NULL	phosphorylation of	tyrosine		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29908	12	7414	7	NULL	NULL	0	NULL	bradykinin receptor	NULL		induce	NULL	rapidly			Shc	NULL	phosphorylation of	tyrosine		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29909	13	7414	7	NULL	NULL	0	NULL	lysophosphatidic acid receptor	NULL		induce	NULL	rapidly			Shc-Grb2 complexes	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29910	14	7414	7	NULL	NULL	0	NULL	thyroid-releasing hormone receptor	NULL		induce	NULL	rapidly			Shc-Grb2 complexes	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29911	15	7414	7	NULL	NULL	0	NULL	endothelin-1 receptor	NULL		induce	NULL	rapidly			Shc-Grb2 complexes	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29912	16	7414	7	NULL	NULL	0	NULL	bradykinin receptor	NULL		induce	NULL	rapidly			Shc-Grb2 complexes	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29913	18	7414	7	NULL	NULL	0	NULL	statement 17	NULL		activates	NULL				Ras	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29914	17	7414	7	NULL	NULL	0	NULL	GPCR	NULL		couple with	NULL				RTK	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29915	19	7414	7	NULL	NULL	0	NULL	lysophosphatidic acid receptor	NULL		is a type of	NULL				GPCR	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29916	20	7414	7	NULL	NULL	0	NULL	thyroid-releasing hormone receptor	NULL		is a type of	NULL				GPCR	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29917	21	7414	7	NULL	NULL	0	NULL	endothelin-1 receptor	NULL		is a type of	NULL				GPCR	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
29918	22	7414	7	NULL	NULL	0	NULL	bradykinin receptor	NULL		is a type of	NULL				GPCR	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_994_s_175	12714438	25 MAPKs link external signals to nuclear responses, such as gene expression in response to growth factor binding to either RTK or GPCR. 26,27  The action of Ras in MAPK signal transduction is triggered by activation of Galphaq- or Galphai-coupled GPCRs. 25,28  Stimulation of various GPCRs, such as those for lysophosphatidic acid, 29 thyroid-releasing hormone, 30 endothelin-1, 31 and bradykinin, 32 rapidly induce tyrosine phosphorylation of Shc and formation of Shc-Grb2 complexes, steps that couple both GPCR and RTK to Ras activation.	bind
27730	1	7417	5	13	NULL	NULL	NULL	TNF-alpha	GP		promote					ICAM-1	GP	clustering of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_10_1089_s_234	12714560	25 These results collectively point to an important role of TNF-alpha in promoting ICAM-1 clustering, and the increased binding activity of cell surface ICAM-1 to PMN.	bind
27731	2	7417	5	13	NULL	NULL	NULL	ICAM-1	GP	cell surface	bind					PMN	Cell				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_10_1089_s_234	12714560	25 These results collectively point to an important role of TNF-alpha in promoting ICAM-1 clustering, and the increased binding activity of cell surface ICAM-1 to PMN.	bind
27732	3	7417	5	13	NULL	NULL	NULL	TNF-alpha	GP		increases					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_10_1089_s_234	12714560	25 These results collectively point to an important role of TNF-alpha in promoting ICAM-1 clustering, and the increased binding activity of cell surface ICAM-1 to PMN.	bind
29919	1	7417	7	NULL	NULL	0	NULL	TNF-alpha	NULL		promote	NULL				ICAM-1	NULL	clustering of			NULL		0	NULL	NULL	NULL	gw60_circulationres_92_10_1089_s_234	12714560	25 These results collectively point to an important role of TNF-alpha in promoting ICAM-1 clustering, and the increased binding activity of cell surface ICAM-1 to PMN.	bind
29920	2	7417	7	NULL	NULL	0	NULL	ICAM-1	NULL	cell surface	binds	NULL				PMN	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_92_10_1089_s_234	12714560	25 These results collectively point to an important role of TNF-alpha in promoting ICAM-1 clustering, and the increased binding activity of cell surface ICAM-1 to PMN.	bind
29921	3	7417	7	NULL	NULL	0	NULL	TNF-alpha	NULL		increase	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_92_10_1089_s_234	12714560	25 These results collectively point to an important role of TNF-alpha in promoting ICAM-1 clustering, and the increased binding activity of cell surface ICAM-1 to PMN.	bind
27733	1	7418	5	13	NULL	NULL	NULL	heparin-binding proteins	GP		bind					HS	Chemical				NULL	in biological systems	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1549_s_65	15231514	25 This finding is in accordance with the observation that heparin-binding proteins usually bind HS in biological systems.	bind
29922	1	7418	7	NULL	NULL	0	NULL	heparin-binding proteins	NULL		bind	NULL				HS	NULL				NULL	biological systems	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1549_s_65	15231514	25 This finding is in accordance with the observation that heparin-binding proteins usually bind HS in biological systems.	bind
27734	1	7419	5	13	NULL	NULL	NULL	tau 1	GP		bind					MTs	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1649_s_56	10362789	25 To see the tau bound to MTs, the cells were fixed with cold methanol to wash [[ away cytosolic tau. 26  With ]] this fixation protocol, tau 1 immunoreactivity was almost completely colocalized with MTs (Figure 1, c and d)   .	bind
29923	1	7419	7	NULL	NULL	0	NULL	tau 	NULL		bind	NULL				MTs	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_6_1649_s_56	10362789	25 To see the tau bound to MTs, the cells were fixed with cold methanol to wash [[ away cytosolic tau. 26  With ]] this fixation protocol, tau 1 immunoreactivity was almost completely colocalized with MTs (Figure 1, c and d)   .	bind
27735	1	7420	5	13	NULL	NULL	NULL	Mnk1	GP		bind					ERK2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_12_1218_s_257	14605021	25 Whereas Mnk1 binds both ERK2 and p38 MAPK, Mnk2 interacts strongly only with ERK2.	bind
27736	2	7420	5	13	NULL	NULL	NULL	Mnk1	GP		bind					p38 MAPK	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_12_1218_s_257	14605021	25 Whereas Mnk1 binds both ERK2 and p38 MAPK, Mnk2 interacts strongly only with ERK2.	bind
27737	3	7420	5	13	NULL	NULL	NULL	Mnk2	GP		interacts with		strongly			ERK2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_12_1218_s_257	14605021	25 Whereas Mnk1 binds both ERK2 and p38 MAPK, Mnk2 interacts strongly only with ERK2.	bind
29924	1	7420	7	NULL	NULL	0	NULL	Mnk1	NULL		binds	NULL				ERK2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_93_12_1218_s_257	14605021	25 Whereas Mnk1 binds both ERK2 and p38 MAPK, Mnk2 interacts strongly only with ERK2.	bind
29925	2	7420	7	NULL	NULL	0	NULL	Mnk1	NULL		binds	NULL				p38 MAPK	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_93_12_1218_s_257	14605021	25 Whereas Mnk1 binds both ERK2 and p38 MAPK, Mnk2 interacts strongly only with ERK2.	bind
29926	3	7420	7	NULL	NULL	0	NULL	Mnk2	NULL		interacts	NULL	strongly			ERK2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_93_12_1218_s_257	14605021	25 Whereas Mnk1 binds both ERK2 and p38 MAPK, Mnk2 interacts strongly only with ERK2.	bind
27738	1	7422	5	13	NULL	NULL	NULL	aldosterone	Chemical		bind					MR	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_19_2512_s_27	12756192	25) The binding of aldosterone to the MR results in dissociation of the ligand-activated MR from a multiprotein complex containing molecular chaperones, translocation into the nucleus, and binding to hormone response elements in the regulatory region of target gene promoters.	bind
27739	2	7422	5	13	NULL	NULL	NULL	MR	GP	ligand-activated	froms multiprotein complex with					molecular chaperones	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_19_2512_s_27	12756192	25) The binding of aldosterone to the MR results in dissociation of the ligand-activated MR from a multiprotein complex containing molecular chaperones, translocation into the nucleus, and binding to hormone response elements in the regulatory region of target gene promoters.	bind
27740	3	7422	5	13	NULL	NULL	NULL	statement 1	Process		results in					statement 2	Process	dissociation of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_19_2512_s_27	12756192	25) The binding of aldosterone to the MR results in dissociation of the ligand-activated MR from a multiprotein complex containing molecular chaperones, translocation into the nucleus, and binding to hormone response elements in the regulatory region of target gene promoters.	bind
27741	4	7422	5	13	NULL	NULL	NULL	MR	GP		is translocated to					nucleus	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_19_2512_s_27	12756192	25) The binding of aldosterone to the MR results in dissociation of the ligand-activated MR from a multiprotein complex containing molecular chaperones, translocation into the nucleus, and binding to hormone response elements in the regulatory region of target gene promoters.	bind
27742	5	7422	5	13	NULL	NULL	NULL	statement 1	Process		results in					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_19_2512_s_27	12756192	25) The binding of aldosterone to the MR results in dissociation of the ligand-activated MR from a multiprotein complex containing molecular chaperones, translocation into the nucleus, and binding to hormone response elements in the regulatory region of target gene promoters.	bind
27743	6	7422	5	13	NULL	NULL	NULL	MR	GP		bind					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_19_2512_s_27	12756192	25) The binding of aldosterone to the MR results in dissociation of the ligand-activated MR from a multiprotein complex containing molecular chaperones, translocation into the nucleus, and binding to hormone response elements in the regulatory region of target gene promoters.	bind
27744	7	7422	5	13	NULL	NULL	NULL	statement 1	Process		results in					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_19_2512_s_27	12756192	25) The binding of aldosterone to the MR results in dissociation of the ligand-activated MR from a multiprotein complex containing molecular chaperones, translocation into the nucleus, and binding to hormone response elements in the regulatory region of target gene promoters.	bind
54503	8	7422	5	13	NULL	NULL	NULL	target gene	NucleicAcid		resides in				hormone response elements	target gene	NucleicAcid			regulatory region of promoter	NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_19_2512_s_27	12756192	25) The binding of aldosterone to the MR results in dissociation of the ligand-activated MR from a multiprotein complex containing molecular chaperones, translocation into the nucleus, and binding to hormone response elements in the regulatory region of target gene promoters.	bind
29927	1	7422	7	NULL	NULL	0	NULL	aldosterone	NULL		bind	NULL				MR	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_107_19_2512_s_27	12756192	25) The binding of aldosterone to the MR results in dissociation of the ligand-activated MR from a multiprotein complex containing molecular chaperones, translocation into the nucleus, and binding to hormone response elements in the regulatory region of target gene promoters.	bind
29928	2	7422	7	10	NULL	0	NULL	MR	NULL	ligand-activated	forms multiprotein complex with	NULL				molecular chaperones	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_19_2512_s_27	12756192	25) The binding of aldosterone to the MR results in dissociation of the ligand-activated MR from a multiprotein complex containing molecular chaperones, translocation into the nucleus, and binding to hormone response elements in the regulatory region of target gene promoters.	bind
29929	3	7422	7	NULL	NULL	0	NULL	statement 1	NULL		results in	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_107_19_2512_s_27	12756192	25) The binding of aldosterone to the MR results in dissociation of the ligand-activated MR from a multiprotein complex containing molecular chaperones, translocation into the nucleus, and binding to hormone response elements in the regulatory region of target gene promoters.	bind
29930	4	7422	7	10	NULL	0	NULL	MR			is translocated to					nucleus					NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_19_2512_s_27	12756192	25) The binding of aldosterone to the MR results in dissociation of the ligand-activated MR from a multiprotein complex containing molecular chaperones, translocation into the nucleus, and binding to hormone response elements in the regulatory region of target gene promoters.	bind
29931	5	7422	7	10	NULL	0	NULL	statement 1			bind					statement 7					NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_19_2512_s_27	12756192	25) The binding of aldosterone to the MR results in dissociation of the ligand-activated MR from a multiprotein complex containing molecular chaperones, translocation into the nucleus, and binding to hormone response elements in the regulatory region of target gene promoters.	bind
54502	6	7422	7	10	NULL	0	NULL	statement 1			results in					statement 4					NULL		0	NULL	NULL	NULL	gw70_circulation_107_19_2512_s_27	12756192	25) The binding of aldosterone to the MR results in dissociation of the ligand-activated MR from a multiprotein complex containing molecular chaperones, translocation into the nucleus, and binding to hormone response elements in the regulatory region of target gene promoters.	bind
54504	7	7422	7	10	NULL	0	NULL	target gene			resides in				hormone response elements	target gene				regulatory region of promoter	NULL		0	NULL	NULL	NULL	gw70_circulation_107_19_2512_s_27	12756192	25) The binding of aldosterone to the MR results in dissociation of the ligand-activated MR from a multiprotein complex containing molecular chaperones, translocation into the nucleus, and binding to hormone response elements in the regulatory region of target gene promoters.	bind
27745	1	7424	5	13	NULL	NULL	NULL	AP-2	GP		bind		may			statement 6	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_6_682_s_195	11934836	25, 38 These along with other factors (such as AP-2, CRE, ER, GATA-1, and SP-1) may bind onto  cis elements of known consensus sequences on the human eNOS promoter.	bind
27746	2	7424	5	13	NULL	NULL	NULL	CRE	GP		bind		may			statement 6	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_6_682_s_195	11934836	25, 38 These along with other factors (such as AP-2, CRE, ER, GATA-1, and SP-1) may bind onto  cis elements of known consensus sequences on the human eNOS promoter.	bind
27747	3	7424	5	13	NULL	NULL	NULL	ER	GP		bind		may			statement 6	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_6_682_s_195	11934836	25, 38 These along with other factors (such as AP-2, CRE, ER, GATA-1, and SP-1) may bind onto  cis elements of known consensus sequences on the human eNOS promoter.	bind
27748	4	7424	5	13	NULL	NULL	NULL	GATA-1	GP		bind		may			statement 6	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_6_682_s_195	11934836	25, 38 These along with other factors (such as AP-2, CRE, ER, GATA-1, and SP-1) may bind onto  cis elements of known consensus sequences on the human eNOS promoter.	bind
27749	5	7424	5	13	NULL	NULL	NULL	SP-1	GP		bind		may			statement 6	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_6_682_s_195	11934836	25, 38 These along with other factors (such as AP-2, CRE, ER, GATA-1, and SP-1) may bind onto  cis elements of known consensus sequences on the human eNOS promoter.	bind
54508	6	7424	5	13	NULL	NULL	NULL				is present on				cis elements	eNOS	NucleicAcid	human		promoter	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_6_682_s_195	11934836	25, 38 These along with other factors (such as AP-2, CRE, ER, GATA-1, and SP-1) may bind onto  cis elements of known consensus sequences on the human eNOS promoter.	bind
29938	1	7424	7	10	NULL	0	NULL	AP-2			bind		may			statement 6					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_6_682_s_195	11934836	25, 38 These along with other factors (such as AP-2, CRE, ER, GATA-1, and SP-1) may bind onto  cis elements of known consensus sequences on the human eNOS promoter.	bind
29939	2	7424	7	10	NULL	0	NULL	 CRE			bind		may			statement 6					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_6_682_s_195	11934836	25, 38 These along with other factors (such as AP-2, CRE, ER, GATA-1, and SP-1) may bind onto  cis elements of known consensus sequences on the human eNOS promoter.	bind
29940	3	7424	7	10	NULL	0	NULL	ER			bind		may			statement 6					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_6_682_s_195	11934836	25, 38 These along with other factors (such as AP-2, CRE, ER, GATA-1, and SP-1) may bind onto  cis elements of known consensus sequences on the human eNOS promoter.	bind
29941	4	7424	7	10	NULL	0	NULL	GATA-1			bind		may			statement 6					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_6_682_s_195	11934836	25, 38 These along with other factors (such as AP-2, CRE, ER, GATA-1, and SP-1) may bind onto  cis elements of known consensus sequences on the human eNOS promoter.	bind
29942	5	7424	7	10	NULL	0	NULL	SP-1			bind		may			statement 6					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_6_682_s_195	11934836	25, 38 These along with other factors (such as AP-2, CRE, ER, GATA-1, and SP-1) may bind onto  cis elements of known consensus sequences on the human eNOS promoter.	bind
54509	6	7424	7	10	NULL	0	NULL				is present on				cis elements	eNOS		human		promoter	NULL		0	NULL	NULL	NULL	gw60_circulationres_90_6_682_s_195	11934836	25, 38 These along with other factors (such as AP-2, CRE, ER, GATA-1, and SP-1) may bind onto  cis elements of known consensus sequences on the human eNOS promoter.	bind
27750	1	7425	5	13	NULL	NULL	NULL	cytochrome C	GP		enters into					cytosol	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2178_s_26	14551153	25,26  On entry into the cytosol, cytochrome C binds the caspase-activating protein Apaf-1, stimulating its binding to procaspase 9 and activating caspase networks that trigger apoptosis.	bind
27751	2	7425	5	13	NULL	NULL	NULL	cytochrome C	GP		bind					Apaf-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2178_s_26	14551153	25,26  On entry into the cytosol, cytochrome C binds the caspase-activating protein Apaf-1, stimulating its binding to procaspase 9 and activating caspase networks that trigger apoptosis.	bind
27752	3	7425	5	13	NULL	NULL	NULL	Apaf-1	GP		is a type of					caspase-activating protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2178_s_26	14551153	25,26  On entry into the cytosol, cytochrome C binds the caspase-activating protein Apaf-1, stimulating its binding to procaspase 9 and activating caspase networks that trigger apoptosis.	bind
27753	4	7425	5	13	NULL	NULL	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2178_s_26	14551153	25,26  On entry into the cytosol, cytochrome C binds the caspase-activating protein Apaf-1, stimulating its binding to procaspase 9 and activating caspase networks that trigger apoptosis.	bind
27754	5	7425	5	13	NULL	NULL	NULL	Apaf-1	GP		bind					procaspase 9	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2178_s_26	14551153	25,26  On entry into the cytosol, cytochrome C binds the caspase-activating protein Apaf-1, stimulating its binding to procaspase 9 and activating caspase networks that trigger apoptosis.	bind
27755	6	7425	5	13	NULL	NULL	NULL	statement 2	Process		stimulates					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2178_s_26	14551153	25,26  On entry into the cytosol, cytochrome C binds the caspase-activating protein Apaf-1, stimulating its binding to procaspase 9 and activating caspase networks that trigger apoptosis.	bind
27756	7	7425	5	13	NULL	NULL	NULL	statement 6	Process		activates					caspase networks	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2178_s_26	14551153	25,26  On entry into the cytosol, cytochrome C binds the caspase-activating protein Apaf-1, stimulating its binding to procaspase 9 and activating caspase networks that trigger apoptosis.	bind
27757	8	7425	5	13	NULL	NULL	NULL	statement 7	Process		triggers					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2178_s_26	14551153	25,26  On entry into the cytosol, cytochrome C binds the caspase-activating protein Apaf-1, stimulating its binding to procaspase 9 and activating caspase networks that trigger apoptosis.	bind
29943	1	7425	7	NULL	NULL	0	NULL	 cytochrome C	NULL		binds	NULL				Apaf-1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2178_s_26	14551153	25,26  On entry into the cytosol, cytochrome C binds the caspase-activating protein Apaf-1, stimulating its binding to procaspase 9 and activating caspase networks that trigger apoptosis.	bind
29944	2	7425	7	NULL	NULL	0	NULL	statement 1	NULL		occurs upon	NULL				cytosol	NULL	entry into the			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2178_s_26	14551153	25,26  On entry into the cytosol, cytochrome C binds the caspase-activating protein Apaf-1, stimulating its binding to procaspase 9 and activating caspase networks that trigger apoptosis.	bind
29945	3	7425	7	NULL	NULL	0	NULL	Apaf-1	NULL		is a type of	NULL				caspase-activating protein	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2178_s_26	14551153	25,26  On entry into the cytosol, cytochrome C binds the caspase-activating protein Apaf-1, stimulating its binding to procaspase 9 and activating caspase networks that trigger apoptosis.	bind
29946	4	7425	7	NULL	NULL	0	NULL	cytochrome C	NULL		binds	NULL				procaspase 9	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2178_s_26	14551153	25,26  On entry into the cytosol, cytochrome C binds the caspase-activating protein Apaf-1, stimulating its binding to procaspase 9 and activating caspase networks that trigger apoptosis.	bind
29947	5	7425	7	NULL	NULL	0	NULL	statement 1	NULL		stimulates	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2178_s_26	14551153	25,26  On entry into the cytosol, cytochrome C binds the caspase-activating protein Apaf-1, stimulating its binding to procaspase 9 and activating caspase networks that trigger apoptosis.	bind
29948	6	7425	7	NULL	NULL	0	NULL	statement 5	NULL		activate	NULL				caspase networks	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2178_s_26	14551153	25,26  On entry into the cytosol, cytochrome C binds the caspase-activating protein Apaf-1, stimulating its binding to procaspase 9 and activating caspase networks that trigger apoptosis.	bind
29949	7	7425	7	NULL	NULL	0	NULL	statement 6	NULL		trigger	NULL				apoptosis	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2178_s_26	14551153	25,26  On entry into the cytosol, cytochrome C binds the caspase-activating protein Apaf-1, stimulating its binding to procaspase 9 and activating caspase networks that trigger apoptosis.	bind
27758	1	7426	5	13	NULL	NULL	NULL	25-Dx	GP		is a variant of					IZA	GP				NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_316_1_448_s_19	16234411	25-Dx is a variant of IZA (Min et al., 2004 ), suggesting that it binds to heme, and we show in the present study that Hpr6 binds to heme.	bind
27759	2	7426	5	13	NULL	NULL	NULL	25-Dx	GP		bind					heme	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_316_1_448_s_19	16234411	25-Dx is a variant of IZA (Min et al., 2004 ), suggesting that it binds to heme, and we show in the present study that Hpr6 binds to heme.	bind
27760	3	7426	5	13	NULL	NULL	NULL	statement 1	Process		suggests					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_316_1_448_s_19	16234411	25-Dx is a variant of IZA (Min et al., 2004 ), suggesting that it binds to heme, and we show in the present study that Hpr6 binds to heme.	bind
27761	4	7426	5	13	NULL	NULL	NULL	Hpr6	GP		bind					heme	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_316_1_448_s_19	16234411	25-Dx is a variant of IZA (Min et al., 2004 ), suggesting that it binds to heme, and we show in the present study that Hpr6 binds to heme.	bind
29950	1	7426	7	NULL	NULL	0	NULL	25-Dx	NULL		is a variant of	NULL				IZA	NULL				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_316_1_448_s_19	16234411	25-Dx is a variant of IZA (Min et al., 2004 ), suggesting that it binds to heme, and we show in the present study that Hpr6 binds to heme.	bind
29951	2	7426	7	NULL	NULL	0	NULL	25-Dx	NULL		binds to	NULL				heme	NULL				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_316_1_448_s_19	16234411	25-Dx is a variant of IZA (Min et al., 2004 ), suggesting that it binds to heme, and we show in the present study that Hpr6 binds to heme.	bind
29952	3	7426	7	NULL	NULL	0	NULL	Hpr6	NULL		binds to	NULL				heme	NULL				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_316_1_448_s_19	16234411	25-Dx is a variant of IZA (Min et al., 2004 ), suggesting that it binds to heme, and we show in the present study that Hpr6 binds to heme.	bind
27762	1	7427	5	13	NULL	NULL	NULL	Sp1	GP		is a type of					transcription facor	GP				NULL		NULL	NULL	NULL	NULL	gw60_atherosclerosis_158_1_61_s_202	11500175	25-hydroxycholesterol and Oxidized LDL increased the binding of the transcription facors Sp1 and Sp3 to the TNF-  promoter	bind
27763	2	7427	5	13	NULL	NULL	NULL	Sp3	GP		is a type of					transcription facor	GP				NULL		NULL	NULL	NULL	NULL	gw60_atherosclerosis_158_1_61_s_202	11500175	25-hydroxycholesterol and Oxidized LDL increased the binding of the transcription facors Sp1 and Sp3 to the TNF-  promoter	bind
27764	3	7427	5	13	NULL	NULL	NULL	Sp1	GP		bind					TNF	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_atherosclerosis_158_1_61_s_202	11500175	25-hydroxycholesterol and Oxidized LDL increased the binding of the transcription facors Sp1 and Sp3 to the TNF-  promoter	bind
27765	4	7427	5	13	NULL	NULL	NULL	Sp3	GP		bind					TNF	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_atherosclerosis_158_1_61_s_202	11500175	25-hydroxycholesterol and Oxidized LDL increased the binding of the transcription facors Sp1 and Sp3 to the TNF-  promoter	bind
27766	5	7427	5	13	NULL	NULL	NULL	25-hydroxycholesterol	Chemical		increases					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_atherosclerosis_158_1_61_s_202	11500175	25-hydroxycholesterol and Oxidized LDL increased the binding of the transcription facors Sp1 and Sp3 to the TNF-  promoter	bind
27767	6	7427	5	13	NULL	NULL	NULL	25-hydroxycholesterol	Chemical		increases					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_atherosclerosis_158_1_61_s_202	11500175	25-hydroxycholesterol and Oxidized LDL increased the binding of the transcription facors Sp1 and Sp3 to the TNF-  promoter	bind
27768	7	7427	5	13	NULL	NULL	NULL	LDL	GP	oxidized	increases					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_atherosclerosis_158_1_61_s_202	11500175	25-hydroxycholesterol and Oxidized LDL increased the binding of the transcription facors Sp1 and Sp3 to the TNF-  promoter	bind
27769	8	7427	5	13	NULL	NULL	NULL	LDL	GP	oxidized	increases					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_atherosclerosis_158_1_61_s_202	11500175	25-hydroxycholesterol and Oxidized LDL increased the binding of the transcription facors Sp1 and Sp3 to the TNF-  promoter	bind
29953	1	7427	7	NULL	NULL	0	NULL	Sp1	NULL		bind	NULL				TNF	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_atherosclerosis_158_1_61_s_202	11500175	25-hydroxycholesterol and Oxidized LDL increased the binding of the transcription facors Sp1 and Sp3 to the TNF-  promoter	bind
29954	2	7427	7	NULL	NULL	0	NULL	Sp3	NULL		bind	NULL				TNF	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_atherosclerosis_158_1_61_s_202	11500175	25-hydroxycholesterol and Oxidized LDL increased the binding of the transcription facors Sp1 and Sp3 to the TNF-  promoter	bind
29955	3	7427	7	NULL	NULL	0	NULL	25-hydroxycholesterol	NULL		increase	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_atherosclerosis_158_1_61_s_202	11500175	25-hydroxycholesterol and Oxidized LDL increased the binding of the transcription facors Sp1 and Sp3 to the TNF-  promoter	bind
29956	4	7427	7	NULL	NULL	0	NULL	LDL	NULL	Oxidized	increase	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_atherosclerosis_158_1_61_s_202	11500175	25-hydroxycholesterol and Oxidized LDL increased the binding of the transcription facors Sp1 and Sp3 to the TNF-  promoter	bind
29957	5	7427	7	NULL	NULL	0	NULL	25-hydroxycholesterol	NULL		increase	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_atherosclerosis_158_1_61_s_202	11500175	25-hydroxycholesterol and Oxidized LDL increased the binding of the transcription facors Sp1 and Sp3 to the TNF-  promoter	bind
29958	6	7427	7	NULL	NULL	0	NULL	LDL	NULL	Oxidized	increase	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_atherosclerosis_158_1_61_s_202	11500175	25-hydroxycholesterol and Oxidized LDL increased the binding of the transcription facors Sp1 and Sp3 to the TNF-  promoter	bind
29959	7	7427	7	NULL	NULL	0	NULL	Sp1	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_atherosclerosis_158_1_61_s_202	11500175	25-hydroxycholesterol and Oxidized LDL increased the binding of the transcription facors Sp1 and Sp3 to the TNF-  promoter	bind
29960	8	7427	7	NULL	NULL	0	NULL	Sp3	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_atherosclerosis_158_1_61_s_202	11500175	25-hydroxycholesterol and Oxidized LDL increased the binding of the transcription facors Sp1 and Sp3 to the TNF-  promoter	bind
27770	1	7432	5	13	NULL	NULL	NULL				regulates				SBE	SM22alpha	GP	activity of		promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_circulationres_97_10_983_s_172	16224064	25a,26  In this report, we show that SBE is another critical element regulating SM22alpha promoter activity in vivo, and Smad3 binds to the SBE in response to TGF-beta1 stimulation.	bind
27771	2	7432	5	13	NULL	NULL	NULL	Smad3	GP		bind									SBE	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_10_983_s_172	16224064	25a,26  In this report, we show that SBE is another critical element regulating SM22alpha promoter activity in vivo, and Smad3 binds to the SBE in response to TGF-beta1 stimulation.	bind
27772	3	7432	5	13	NULL	NULL	NULL	TGF-beta1	GP	stimulation	leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_10_983_s_172	16224064	25a,26  In this report, we show that SBE is another critical element regulating SM22alpha promoter activity in vivo, and Smad3 binds to the SBE in response to TGF-beta1 stimulation.	bind
29961	1	7432	7	10	NULL	0	NULL				regulates				SBE	SM22alpha		activity of		promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_circulationres_97_10_983_s_172	16224064	25a,26  In this report, we show that SBE is another critical element regulating SM22alpha promoter activity in vivo, and Smad3 binds to the SBE in response to TGF-beta1 stimulation.	bind
29962	2	7432	7	NULL	NULL	0	NULL	Smad3	NULL		binds to	NULL					NULL			SBE	NULL		0	NULL	NULL	NULL	gw70_circulationres_97_10_983_s_172	16224064	25a,26  In this report, we show that SBE is another critical element regulating SM22alpha promoter activity in vivo, and Smad3 binds to the SBE in response to TGF-beta1 stimulation.	bind
29963	3	7432	7	NULL	NULL	0	NULL	statement 2	NULL		occurs upon	NULL				TGF-beta1	NULL	stimulation of			NULL		0	NULL	NULL	NULL	gw70_circulationres_97_10_983_s_172	16224064	25a,26  In this report, we show that SBE is another critical element regulating SM22alpha promoter activity in vivo, and Smad3 binds to the SBE in response to TGF-beta1 stimulation.	bind
27773	1	7433	5	13	NULL	NULL	NULL	plasmid ColIb-P9 antisense Inc RNA	NucleicAcid		bind					target RNA	NucleicAcid			5''-rUUGGCG-3'' motif in loop sequence	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_5_1034_s_412	11222752	26       Asano,K., Niimi,T., Yokoyama,S. and Mizobuchi,K. (1998) Structural basis for binding of the plasmid ColIb-P9 antisense Inc RNA to its target RNA with the 5''-rUUGGCG-3'' motif in the loop sequence.	bind
29964	1	7433	7	10	NULL	0	NULL	plasmid ColIb-P9 ColIb-P9 antisense Inc RNA			binds					RNA				5''-rUUGGCG-3'' motif in the loop sequence	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_5_1034_s_412	11222752	26       Asano,K., Niimi,T., Yokoyama,S. and Mizobuchi,K. (1998) Structural basis for binding of the plasmid ColIb-P9 antisense Inc RNA to its target RNA with the 5''-rUUGGCG-3'' motif in the loop sequence.	bind
27774	1	7434	5	13	NULL	NULL	NULL	PKR	GP		bind		specifically			RNA	NucleicAcid	delta agent genomic			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2535_s_295	11410661	26       Circle,D.A., Neel,O.D., Robertson,H.D., Clarke,P.A. and Mathews,M.B. (1997) Surprising specificity of PKR binding to delta agent genomic RNA.	bind
29966	1	7434	7	10	NULL	0	NULL	PKR			binds					RNA		delta agent genomic			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2535_s_295	11410661	26       Circle,D.A., Neel,O.D., Robertson,H.D., Clarke,P.A. and Mathews,M.B. (1997) Surprising specificity of PKR binding to delta agent genomic RNA.	bind
27775	1	7435	5	13	NULL	NULL	NULL	MyEF-2	GP		bind					MBP	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_17_3197_s_335	10954586	26       Muralidharan,V., Tretiakova,A., Steplewski,A., Haas,S., Amini,S., Johnson,E. and Khalili,K. (1997) Evidence for inhibition of MyEF-2 binding to MBP promoter by MEF-1/Puralpha.	bind
27776	2	7435	5	13	NULL	NULL	NULL	MEF-1/Puralpha	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_17_3197_s_335	10954586	26       Muralidharan,V., Tretiakova,A., Steplewski,A., Haas,S., Amini,S., Johnson,E. and Khalili,K. (1997) Evidence for inhibition of MyEF-2 binding to MBP promoter by MEF-1/Puralpha.	bind
29969	1	7435	7	NULL	NULL	0	NULL	MyEF-2	NULL		bind	NULL				MBP	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_17_3197_s_335	10954586	26       Muralidharan,V., Tretiakova,A., Steplewski,A., Haas,S., Amini,S., Johnson,E. and Khalili,K. (1997) Evidence for inhibition of MyEF-2 binding to MBP promoter by MEF-1/Puralpha.	bind
29970	2	7435	7	NULL	NULL	0	NULL	MEF-1/Puralpha	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_17_3197_s_335	10954586	26       Muralidharan,V., Tretiakova,A., Steplewski,A., Haas,S., Amini,S., Johnson,E. and Khalili,K. (1997) Evidence for inhibition of MyEF-2 binding to MBP promoter by MEF-1/Puralpha.	bind
27777	1	7436	5	13	NULL	NULL	NULL	CUG-binding protein	GP		bind		specifically							UG dinucleotide repeats	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2766_s_267	11433021	26       Takahashi,N., Sasagawa,N., Suzuki,K. and Ishiura,S. (2000) The CUG-binding protein binds specifically to UG dinucleotide repeats in a yeast three-hybrid system.	bind
29971	1	7436	7	10	NULL	0	NULL	CUG-binding protein	NULL		binds	NULL	specifically				NULL			UG dinucleotide repeats	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2766_s_267	11433021	26       Takahashi,N., Sasagawa,N., Suzuki,K. and Ishiura,S. (2000) The CUG-binding protein binds specifically to UG dinucleotide repeats in a yeast three-hybrid system.	bind
27778	1	7437	5	13	NULL	NULL	NULL	early growth response protein	GP		bind					statement 4	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_652_s_372	11160886	26       Yan,Y.-X., Nakagawa,H., Lees,M.-H. and Rustig,A.K. (1997) Transforming growth factor-alpha enhances cyclin D1 transcription through the binding of early growth response protein to a cis-regulatory element in the cyclin D1 promoter.	bind
27779	2	7437	5	13	NULL	NULL	NULL	Transforming growth factor-alpha	GP		enhances					cyclin D1	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_652_s_372	11160886	26       Yan,Y.-X., Nakagawa,H., Lees,M.-H. and Rustig,A.K. (1997) Transforming growth factor-alpha enhances cyclin D1 transcription through the binding of early growth response protein to a cis-regulatory element in the cyclin D1 promoter.	bind
27780	3	7437	5	13	NULL	NULL	NULL	statement 2	Process		occurs through					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_652_s_372	11160886	26       Yan,Y.-X., Nakagawa,H., Lees,M.-H. and Rustig,A.K. (1997) Transforming growth factor-alpha enhances cyclin D1 transcription through the binding of early growth response protein to a cis-regulatory element in the cyclin D1 promoter.	bind
54510	4	7437	5	13	NULL	NULL	NULL				is present in				cis-regulatory element	cyclin D1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_652_s_372	11160886	26       Yan,Y.-X., Nakagawa,H., Lees,M.-H. and Rustig,A.K. (1997) Transforming growth factor-alpha enhances cyclin D1 transcription through the binding of early growth response protein to a cis-regulatory element in the cyclin D1 promoter.	bind
29972	1	7437	7	10	NULL	0	NULL	early growth response protein			bind					statement 4					NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_652_s_372	11160886	26       Yan,Y.-X., Nakagawa,H., Lees,M.-H. and Rustig,A.K. (1997) Transforming growth factor-alpha enhances cyclin D1 transcription through the binding of early growth response protein to a cis-regulatory element in the cyclin D1 promoter.	bind
29973	2	7437	7	NULL	NULL	0	NULL	Transforming growth factor-alpha	NULL		enhances	NULL				 cyclin D1	NULL	transcription of			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_652_s_372	11160886	26       Yan,Y.-X., Nakagawa,H., Lees,M.-H. and Rustig,A.K. (1997) Transforming growth factor-alpha enhances cyclin D1 transcription through the binding of early growth response protein to a cis-regulatory element in the cyclin D1 promoter.	bind
29974	3	7437	7	NULL	NULL	0	NULL	statement 2	NULL		occurs through	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_652_s_372	11160886	26       Yan,Y.-X., Nakagawa,H., Lees,M.-H. and Rustig,A.K. (1997) Transforming growth factor-alpha enhances cyclin D1 transcription through the binding of early growth response protein to a cis-regulatory element in the cyclin D1 promoter.	bind
54512	4	7437	7	10	NULL	0	NULL				is present in				cis-regulatory element	cyclin D1				promoter	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_652_s_372	11160886	26       Yan,Y.-X., Nakagawa,H., Lees,M.-H. and Rustig,A.K. (1997) Transforming growth factor-alpha enhances cyclin D1 transcription through the binding of early growth response protein to a cis-regulatory element in the cyclin D1 promoter.	bind
27781	1	7438	5	13	NULL	NULL	NULL	Ang II	GP		bind					AT1 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_10_2297_s_133	11031218	26  31  Because candesartan reduces maximal Ang II binding to the AT1 receptor, whereas losartan causes a rightward shift in the Ang II dose response without reducing maximal Ang II binding, 31  it is likely that the partial reduction of Ang II - induced PAI-1 expression by losartan 9  was due to incomplete antagonism of the AT1 receptor.	bind
30138	2	7438	5	13	NULL	NULL	NULL	candesartan	Chemical		reduces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_10_2297_s_133	11031218	26  31  Because candesartan reduces maximal Ang II binding to the AT1 receptor, whereas losartan causes a rightward shift in the Ang II dose response without reducing maximal Ang II binding, 31  it is likely that the partial reduction of Ang II - induced PAI-1 expression by losartan 9  was due to incomplete antagonism of the AT1 receptor.	bind
30140	4	7438	5	13	NULL	NULL	NULL	losartan	Chemical		does not reduce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_10_2297_s_133	11031218	26  31  Because candesartan reduces maximal Ang II binding to the AT1 receptor, whereas losartan causes a rightward shift in the Ang II dose response without reducing maximal Ang II binding, 31  it is likely that the partial reduction of Ang II - induced PAI-1 expression by losartan 9  was due to incomplete antagonism of the AT1 receptor.	bind
30141	5	7438	5	13	NULL	NULL	NULL	Ang II	GP		induces					PAI-1	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_10_2297_s_133	11031218	26  31  Because candesartan reduces maximal Ang II binding to the AT1 receptor, whereas losartan causes a rightward shift in the Ang II dose response without reducing maximal Ang II binding, 31  it is likely that the partial reduction of Ang II - induced PAI-1 expression by losartan 9  was due to incomplete antagonism of the AT1 receptor.	bind
30142	6	7438	5	13	NULL	NULL	NULL	losartan 9	Chemical		reduces		partially			statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_10_2297_s_133	11031218	26  31  Because candesartan reduces maximal Ang II binding to the AT1 receptor, whereas losartan causes a rightward shift in the Ang II dose response without reducing maximal Ang II binding, 31  it is likely that the partial reduction of Ang II - induced PAI-1 expression by losartan 9  was due to incomplete antagonism of the AT1 receptor.	bind
30143	7	7438	5	13	NULL	NULL	NULL	AT1 receptor	GP	incomplete antagonism of	leads to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_10_2297_s_133	11031218	26  31  Because candesartan reduces maximal Ang II binding to the AT1 receptor, whereas losartan causes a rightward shift in the Ang II dose response without reducing maximal Ang II binding, 31  it is likely that the partial reduction of Ang II - induced PAI-1 expression by losartan 9  was due to incomplete antagonism of the AT1 receptor.	bind
29975	1	7438	7	NULL	NULL	0	NULL	 Ang II	NULL		bind	NULL				AT1 receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_10_2297_s_133	11031218	26  31  Because candesartan reduces maximal Ang II binding to the AT1 receptor, whereas losartan causes a rightward shift in the Ang II dose response without reducing maximal Ang II binding, 31  it is likely that the partial reduction of Ang II - induced PAI-1 expression by losartan 9  was due to incomplete antagonism of the AT1 receptor.	bind
29976	2	7438	7	NULL	NULL	0	NULL	candesartan	NULL		reduces	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_10_2297_s_133	11031218	26  31  Because candesartan reduces maximal Ang II binding to the AT1 receptor, whereas losartan causes a rightward shift in the Ang II dose response without reducing maximal Ang II binding, 31  it is likely that the partial reduction of Ang II - induced PAI-1 expression by losartan 9  was due to incomplete antagonism of the AT1 receptor.	bind
29977	3	7438	7	NULL	NULL	0	NULL	losartan	NULL		does not reduce	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_10_2297_s_133	11031218	26  31  Because candesartan reduces maximal Ang II binding to the AT1 receptor, whereas losartan causes a rightward shift in the Ang II dose response without reducing maximal Ang II binding, 31  it is likely that the partial reduction of Ang II - induced PAI-1 expression by losartan 9  was due to incomplete antagonism of the AT1 receptor.	bind
29978	4	7438	7	NULL	NULL	0	NULL	Ang II	NULL		induce	NULL				 PAI-1 	NULL	expression of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_10_2297_s_133	11031218	26  31  Because candesartan reduces maximal Ang II binding to the AT1 receptor, whereas losartan causes a rightward shift in the Ang II dose response without reducing maximal Ang II binding, 31  it is likely that the partial reduction of Ang II - induced PAI-1 expression by losartan 9  was due to incomplete antagonism of the AT1 receptor.	bind
29979	5	7438	7	NULL	NULL	0	NULL	losartan	NULL		reduce	NULL	partially			statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_10_2297_s_133	11031218	26  31  Because candesartan reduces maximal Ang II binding to the AT1 receptor, whereas losartan causes a rightward shift in the Ang II dose response without reducing maximal Ang II binding, 31  it is likely that the partial reduction of Ang II - induced PAI-1 expression by losartan 9  was due to incomplete antagonism of the AT1 receptor.	bind
29980	6	7438	7	NULL	NULL	0	NULL	statement 5	NULL		is due to	NULL				AT1 receptor	NULL	incomplete antagonism of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_10_2297_s_133	11031218	26  31  Because candesartan reduces maximal Ang II binding to the AT1 receptor, whereas losartan causes a rightward shift in the Ang II dose response without reducing maximal Ang II binding, 31  it is likely that the partial reduction of Ang II - induced PAI-1 expression by losartan 9  was due to incomplete antagonism of the AT1 receptor.	bind
27782	1	7439	5	13	NULL	NULL	NULL	PBL	Cell		bind					smooth muscle cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_1953_s_251	10595925	26  A 50% reduction of PBL binding to smooth muscle cells with these antibodies was observed.	bind
29981	1	7439	7	NULL	NULL	0	NULL	PBL	NULL		bind	NULL				smooth muscle cells	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_6_1953_s_251	10595925	26  A 50% reduction of PBL binding to smooth muscle cells with these antibodies was observed.	bind
27783	1	7440	5	13	NULL	NULL	NULL	VLA-4	GP		bind					FN	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_2_153_s_38	10904000	26  An alternative interpretation of these results 25  is that the VCAM-1 and FN binding sites may indeed be identical, but the binding affinity of VLA-4 for FN could be lower.	bind
29982	1	7440	7	NULL	NULL	0	NULL	VLA-4	NULL		bind	NULL				FN	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_2_153_s_38	10904000	26  An alternative interpretation of these results 25  is that the VCAM-1 and FN binding sites may indeed be identical, but the binding affinity of VLA-4 for FN could be lower.	bind
27784	1	7441	5	13	NULL	NULL	NULL	ELAM-1	GP		bind					neutrophils	Cell		carbohydrate containing moiety		NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_2_403_s_142	7805244	26  ELAM-1 binds to a carbohydrate containing moiety (sialyl Lewisx structure) on neutrophils, while ICAM-1 binds to the heterodimeric B2 integrins (CD11a/CD18 and CD11b/CD18).	bind
27785	2	7441	5	13	NULL	NULL	NULL	ICAM-1	GP		bind					CD11a/CD18	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_2_403_s_142	7805244	26  ELAM-1 binds to a carbohydrate containing moiety (sialyl Lewisx structure) on neutrophils, while ICAM-1 binds to the heterodimeric B2 integrins (CD11a/CD18 and CD11b/CD18).	bind
27786	3	7441	5	13	NULL	NULL	NULL	ICAM-1	GP		bind					CD11b/CD18	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_2_403_s_142	7805244	26  ELAM-1 binds to a carbohydrate containing moiety (sialyl Lewisx structure) on neutrophils, while ICAM-1 binds to the heterodimeric B2 integrins (CD11a/CD18 and CD11b/CD18).	bind
27787	4	7441	5	13	NULL	NULL	NULL	CD11b/CD18	GP		is a type of					heterodimeric B2 integrins	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_2_403_s_142	7805244	26  ELAM-1 binds to a carbohydrate containing moiety (sialyl Lewisx structure) on neutrophils, while ICAM-1 binds to the heterodimeric B2 integrins (CD11a/CD18 and CD11b/CD18).	bind
27788	5	7441	5	13	NULL	NULL	NULL	CD11a/CD18	GP		is a type of					heterodimeric B2 integrins	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_2_403_s_142	7805244	26  ELAM-1 binds to a carbohydrate containing moiety (sialyl Lewisx structure) on neutrophils, while ICAM-1 binds to the heterodimeric B2 integrins (CD11a/CD18 and CD11b/CD18).	bind
29984	1	7441	7	NULL	NULL	0	NULL	ELAM-1	NULL		binds to	NULL				neutrophils	NULL		carbohydrate containing moiety		NULL		0	NULL	NULL	NULL	gw60_circulation_91_2_403_s_142	7805244	26  ELAM-1 binds to a carbohydrate containing moiety (sialyl Lewisx structure) on neutrophils, while ICAM-1 binds to the heterodimeric B2 integrins (CD11a/CD18 and CD11b/CD18).	bind
29985	2	7441	7	10	NULL	0	NULL	ICAM-1 			binds to					CD11a/CD18					NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_2_403_s_142	7805244	26  ELAM-1 binds to a carbohydrate containing moiety (sialyl Lewisx structure) on neutrophils, while ICAM-1 binds to the heterodimeric B2 integrins (CD11a/CD18 and CD11b/CD18).	bind
54513	3	7441	7	10	NULL	0	NULL	ICAM-1			bind					CD11b/CD18					NULL		0	NULL	NULL	NULL	gw60_circulation_91_2_403_s_142	7805244	26  ELAM-1 binds to a carbohydrate containing moiety (sialyl Lewisx structure) on neutrophils, while ICAM-1 binds to the heterodimeric B2 integrins (CD11a/CD18 and CD11b/CD18).	bind
54514	4	7441	7	10	NULL	0	NULL	CD11b/CD18			is a type of					heterodimeric B2 integrins					NULL		0	NULL	NULL	NULL	gw60_circulation_91_2_403_s_142	7805244	26  ELAM-1 binds to a carbohydrate containing moiety (sialyl Lewisx structure) on neutrophils, while ICAM-1 binds to the heterodimeric B2 integrins (CD11a/CD18 and CD11b/CD18).	bind
54515	5	7441	7	10	NULL	0	NULL	CD11a/CD18			is a type of					heterodimeric B2 integrins					NULL		0	NULL	NULL	NULL	gw60_circulation_91_2_403_s_142	7805244	26  ELAM-1 binds to a carbohydrate containing moiety (sialyl Lewisx structure) on neutrophils, while ICAM-1 binds to the heterodimeric B2 integrins (CD11a/CD18 and CD11b/CD18).	bind
27789	1	7442	5	13	NULL	NULL	NULL	synthetic agonist of retinoic acid	Chemical		bind		selectively			RXR	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_1_4_s_77	8925567	26  Further analysis using synthetic agonists of retinoic acid, which selectively bind to RXR or RAR, were used in  trans-activation transient transfection assays, demonstrating that RAR/RXR heterodimers mediate suppression of alpha-adrenergic receptor-dependent hypertrophy.	bind
27790	2	7442	5	13	NULL	NULL	NULL	synthetic agonist of retinoic acid	Chemical		bind		selectively			RAR	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_1_4_s_77	8925567	26  Further analysis using synthetic agonists of retinoic acid, which selectively bind to RXR or RAR, were used in  trans-activation transient transfection assays, demonstrating that RAR/RXR heterodimers mediate suppression of alpha-adrenergic receptor-dependent hypertrophy.	bind
27791	3	7442	5	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_1_4_s_77	8925567	26  Further analysis using synthetic agonists of retinoic acid, which selectively bind to RXR or RAR, were used in  trans-activation transient transfection assays, demonstrating that RAR/RXR heterodimers mediate suppression of alpha-adrenergic receptor-dependent hypertrophy.	bind
27792	4	7442	5	13	NULL	NULL	NULL	RAR/RXR heterodimers	GP		mediate					hypertrophy	Process	suppression of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_1_4_s_77	8925567	26  Further analysis using synthetic agonists of retinoic acid, which selectively bind to RXR or RAR, were used in  trans-activation transient transfection assays, demonstrating that RAR/RXR heterodimers mediate suppression of alpha-adrenergic receptor-dependent hypertrophy.	bind
27793	5	7442	5	13	NULL	NULL	NULL	hypertrophy	Process		is dependent on					alpha-adrenergic receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_1_4_s_77	8925567	26  Further analysis using synthetic agonists of retinoic acid, which selectively bind to RXR or RAR, were used in  trans-activation transient transfection assays, demonstrating that RAR/RXR heterodimers mediate suppression of alpha-adrenergic receptor-dependent hypertrophy.	bind
29986	1	7442	7	10	NULL	0	NULL	synthetic agonist of retinoic acid			bind		selectively			RXR					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_1_4_s_77	8925567	26  Further analysis using synthetic agonists of retinoic acid, which selectively bind to RXR or RAR, were used in  trans-activation transient transfection assays, demonstrating that RAR/RXR heterodimers mediate suppression of alpha-adrenergic receptor-dependent hypertrophy.	bind
29987	2	7442	7	10	NULL	0	NULL	synthetic agonist of retinoic acid			bind		selectively			RAR					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_1_4_s_77	8925567	26  Further analysis using synthetic agonists of retinoic acid, which selectively bind to RXR or RAR, were used in  trans-activation transient transfection assays, demonstrating that RAR/RXR heterodimers mediate suppression of alpha-adrenergic receptor-dependent hypertrophy.	bind
29988	3	7442	7	10	NULL	0	NULL	RAR/RXR heterodimers			mediate					hypertrophy		suppression of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_1_4_s_77	8925567	26  Further analysis using synthetic agonists of retinoic acid, which selectively bind to RXR or RAR, were used in  trans-activation transient transfection assays, demonstrating that RAR/RXR heterodimers mediate suppression of alpha-adrenergic receptor-dependent hypertrophy.	bind
54516	4	7442	7	10	NULL	0	NULL	hypertrophy			is dependent on					alpha-adrenergic receptor					NULL		0	NULL	NULL	NULL	gw60_circulationres_79_1_4_s_77	8925567	26  Further analysis using synthetic agonists of retinoic acid, which selectively bind to RXR or RAR, were used in  trans-activation transient transfection assays, demonstrating that RAR/RXR heterodimers mediate suppression of alpha-adrenergic receptor-dependent hypertrophy.	bind
54517	5	7442	7	10	NULL	0	NULL	statement 1			is an alternative to					statement 2					NULL		0	NULL	NULL	NULL	gw60_circulationres_79_1_4_s_77	8925567	26  Further analysis using synthetic agonists of retinoic acid, which selectively bind to RXR or RAR, were used in  trans-activation transient transfection assays, demonstrating that RAR/RXR heterodimers mediate suppression of alpha-adrenergic receptor-dependent hypertrophy.	bind
27794	1	7443	5	13	NULL	NULL	NULL	NF-kappaB	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_82_5_576_s_238	9529162	26  In contrast, cells subjected to more severe hypoxia (0% O2 for 1 to 6 hours) exhibited time-dependent increases in the DNA binding activities of both NF-kappaB and AP-1 as shown by gel shift analysis (Figs 7A   and 7B  ).	bind
27795	2	7443	5	13	NULL	NULL	NULL	AP-1	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_82_5_576_s_238	9529162	26  In contrast, cells subjected to more severe hypoxia (0% O2 for 1 to 6 hours) exhibited time-dependent increases in the DNA binding activities of both NF-kappaB and AP-1 as shown by gel shift analysis (Figs 7A   and 7B  ).	bind
29989	1	7443	7	NULL	NULL	0	NULL	NF-kappaB	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_82_5_576_s_238	9529162	26  In contrast, cells subjected to more severe hypoxia (0% O2 for 1 to 6 hours) exhibited time-dependent increases in the DNA binding activities of both NF-kappaB and AP-1 as shown by gel shift analysis (Figs 7A   and 7B  ).	bind
29990	2	7443	7	NULL	NULL	0	NULL	AP-1	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_82_5_576_s_238	9529162	26  In contrast, cells subjected to more severe hypoxia (0% O2 for 1 to 6 hours) exhibited time-dependent increases in the DNA binding activities of both NF-kappaB and AP-1 as shown by gel shift analysis (Figs 7A   and 7B  ).	bind
28033	1	7444	5	13	NULL	NULL	NULL	protein(s)	GP		bind					ecNOS	GP	putative		NF-1 binding site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_8_1255_s_218	7543000	26  In gel mobility shift assays, a polyclonal antibody against CTF/NF-1 crossreacted with the protein(s) bound to the putative NF-1 binding site of the ecNOS promoter, whereas they had low affinity for consensus NF-1 oligonucleotides.	bind
28034	2	7444	5	13	NULL	NULL	NULL	CTF/NF-1 polyclonal antibody	GP		crossreacts with					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_8_1255_s_218	7543000	26  In gel mobility shift assays, a polyclonal antibody against CTF/NF-1 crossreacted with the protein(s) bound to the putative NF-1 binding site of the ecNOS promoter, whereas they had low affinity for consensus NF-1 oligonucleotides.	bind
28035	3	7444	5	13	NULL	NULL	NULL	CTF/NF-1 polyclonal antibody	GP		bind		low affinity			NF-1 oligonucleotides	NucleicAcid	consensus			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_8_1255_s_218	7543000	26  In gel mobility shift assays, a polyclonal antibody against CTF/NF-1 crossreacted with the protein(s) bound to the putative NF-1 binding site of the ecNOS promoter, whereas they had low affinity for consensus NF-1 oligonucleotides.	bind
29991	1	7444	7	10	NULL	0	NULL	 proteins			bind					ecNOS		putative		NF-1 binding site in promoter	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_8_1255_s_218	7543000	26  In gel mobility shift assays, a polyclonal antibody against CTF/NF-1 crossreacted with the protein(s) bound to the putative NF-1 binding site of the ecNOS promoter, whereas they had low affinity for consensus NF-1 oligonucleotides.	bind
29992	2	7444	7	NULL	NULL	0	NULL	CTF/NF-1 polyclonal antibody	NULL		crossreacts with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_8_1255_s_218	7543000	26  In gel mobility shift assays, a polyclonal antibody against CTF/NF-1 crossreacted with the protein(s) bound to the putative NF-1 binding site of the ecNOS promoter, whereas they had low affinity for consensus NF-1 oligonucleotides.	bind
29993	3	7444	7	NULL	NULL	0	NULL	CTF/NF-1 polyclonal antibody	NULL		bind	NULL	low affinity			 NF-1 oligonucleotides	NULL	consensus			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_8_1255_s_218	7543000	26  In gel mobility shift assays, a polyclonal antibody against CTF/NF-1 crossreacted with the protein(s) bound to the putative NF-1 binding site of the ecNOS promoter, whereas they had low affinity for consensus NF-1 oligonucleotides.	bind
28036	1	7445	5	13	NULL	NULL	NULL	prothrombin	GP		bind					CMs	CellComponent	native;;chyle			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_1_33_s_139	9445253	26  In our previous studies, we examined binding of prothrombin to native chyle CMs, which contain more phospholipids and a higher proportion of phosphatidylethanolamine in the polar surface coat 49  than the particles that have been exposed to plasma or lipoprotein lipase.	bind
28037	2	7445	5	13	NULL	NULL	NULL	CMs	CellComponent	native;;chyle	contains					phospholipids	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_1_33_s_139	9445253	26  In our previous studies, we examined binding of prothrombin to native chyle CMs, which contain more phospholipids and a higher proportion of phosphatidylethanolamine in the polar surface coat 49  than the particles that have been exposed to plasma or lipoprotein lipase.	bind
28038	3	7445	5	13	NULL	NULL	NULL	CMs	CellComponent	native;;chyle	contains					phosphatidylethanolamine	Chemical	higher proportion of			NULL	polar surface coat	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_1_33_s_139	9445253	26  In our previous studies, we examined binding of prothrombin to native chyle CMs, which contain more phospholipids and a higher proportion of phosphatidylethanolamine in the polar surface coat 49  than the particles that have been exposed to plasma or lipoprotein lipase.	bind
29994	1	7445	7	10	NULL	0	NULL	prothrombin			binds					CMs		native;;chyle			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_1_33_s_139	9445253	26  In our previous studies, we examined binding of prothrombin to native chyle CMs, which contain more phospholipids and a higher proportion of phosphatidylethanolamine in the polar surface coat 49  than the particles that have been exposed to plasma or lipoprotein lipase.	bind
29995	2	7445	7	10	NULL	0	NULL	CMs		native;;chyle	contains					phospholipids					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_1_33_s_139	9445253	26  In our previous studies, we examined binding of prothrombin to native chyle CMs, which contain more phospholipids and a higher proportion of phosphatidylethanolamine in the polar surface coat 49  than the particles that have been exposed to plasma or lipoprotein lipase.	bind
29996	3	7445	7	10	NULL	0	NULL	CMs		native;;chyle	contains					phosphatidylethanolamine 					NULL	polar surface coat	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_1_33_s_139	9445253	26  In our previous studies, we examined binding of prothrombin to native chyle CMs, which contain more phospholipids and a higher proportion of phosphatidylethanolamine in the polar surface coat 49  than the particles that have been exposed to plasma or lipoprotein lipase.	bind
30113	1	7446	5	13	NULL	NULL	NULL	thrombin	GP		bind					clot					NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_7_681_s_134	9495304	26  The superior antithrombotic efficacy of specific thrombin inhibition over heparin appears to be due to several mechanisms, including better inhibition of catalytically active clot-bound thrombin, 27  28  lack of natural inhibitors against hirudin but present against heparin, 29  30  and high affinity for platelet thrombin receptor by r-hirudin, which can displace thrombin bound to platelet receptor.	bind
30114	8	7446	5	13	NULL	NULL	NULL	statement 1	Process	inhibition of;;catalytically active	results in					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_7_681_s_134	9495304	26  The superior antithrombotic efficacy of specific thrombin inhibition over heparin appears to be due to several mechanisms, including better inhibition of catalytically active clot-bound thrombin, 27  28  lack of natural inhibitors against hirudin but present against heparin, 29  30  and high affinity for platelet thrombin receptor by r-hirudin, which can displace thrombin bound to platelet receptor.	bind
30115	3	7446	5	13	NULL	NULL	NULL	inhibitors	Chemical	natural	is present against					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_7_681_s_134	9495304	26  The superior antithrombotic efficacy of specific thrombin inhibition over heparin appears to be due to several mechanisms, including better inhibition of catalytically active clot-bound thrombin, 27  28  lack of natural inhibitors against hirudin but present against heparin, 29  30  and high affinity for platelet thrombin receptor by r-hirudin, which can displace thrombin bound to platelet receptor.	bind
30117	5	7446	5	13	NULL	NULL	NULL	r-hirudin	GP		bind		high affinity			platelet thrombin receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_7_681_s_134	9495304	26  The superior antithrombotic efficacy of specific thrombin inhibition over heparin appears to be due to several mechanisms, including better inhibition of catalytically active clot-bound thrombin, 27  28  lack of natural inhibitors against hirudin but present against heparin, 29  30  and high affinity for platelet thrombin receptor by r-hirudin, which can displace thrombin bound to platelet receptor.	bind
30118	6	7446	5	13	NULL	NULL	NULL	thrombin	GP		bind					platelet receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_7_681_s_134	9495304	26  The superior antithrombotic efficacy of specific thrombin inhibition over heparin appears to be due to several mechanisms, including better inhibition of catalytically active clot-bound thrombin, 27  28  lack of natural inhibitors against hirudin but present against heparin, 29  30  and high affinity for platelet thrombin receptor by r-hirudin, which can displace thrombin bound to platelet receptor.	bind
30119	7	7446	5	13	NULL	NULL	NULL	statement 5	Process		displaces					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_7_681_s_134	9495304	26  The superior antithrombotic efficacy of specific thrombin inhibition over heparin appears to be due to several mechanisms, including better inhibition of catalytically active clot-bound thrombin, 27  28  lack of natural inhibitors against hirudin but present against heparin, 29  30  and high affinity for platelet thrombin receptor by r-hirudin, which can displace thrombin bound to platelet receptor.	bind
30122	2	7446	5	13	NULL	NULL	NULL	thrombin	GP	antithrombotic efficacy of;;inhibition of	is superior to					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_7_681_s_134	9495304	26  The superior antithrombotic efficacy of specific thrombin inhibition over heparin appears to be due to several mechanisms, including better inhibition of catalytically active clot-bound thrombin, 27  28  lack of natural inhibitors against hirudin but present against heparin, 29  30  and high affinity for platelet thrombin receptor by r-hirudin, which can displace thrombin bound to platelet receptor.	bind
54518	4	7446	5	13	NULL	NULL	NULL	statement 3	Process		results in					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_7_681_s_134	9495304	26  The superior antithrombotic efficacy of specific thrombin inhibition over heparin appears to be due to several mechanisms, including better inhibition of catalytically active clot-bound thrombin, 27  28  lack of natural inhibitors against hirudin but present against heparin, 29  30  and high affinity for platelet thrombin receptor by r-hirudin, which can displace thrombin bound to platelet receptor.	bind
54519	9	7446	5	13	NULL	NULL	NULL	statement 5	Process		results in					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_7_681_s_134	9495304	26  The superior antithrombotic efficacy of specific thrombin inhibition over heparin appears to be due to several mechanisms, including better inhibition of catalytically active clot-bound thrombin, 27  28  lack of natural inhibitors against hirudin but present against heparin, 29  30  and high affinity for platelet thrombin receptor by r-hirudin, which can displace thrombin bound to platelet receptor.	bind
29998	1	7446	7	NULL	NULL	0	NULL	thrombin 	NULL		bind	NULL				platelet receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_97_7_681_s_134	9495304	26  The superior antithrombotic efficacy of specific thrombin inhibition over heparin appears to be due to several mechanisms, including better inhibition of catalytically active clot-bound thrombin, 27  28  lack of natural inhibitors against hirudin but present against heparin, 29  30  and high affinity for platelet thrombin receptor by r-hirudin, which can displace thrombin bound to platelet receptor.	bind
30000	2	7446	7	NULL	NULL	0	NULL	 r-hirudin	NULL		high affinity for	NULL				platelet thrombin receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_97_7_681_s_134	9495304	26  The superior antithrombotic efficacy of specific thrombin inhibition over heparin appears to be due to several mechanisms, including better inhibition of catalytically active clot-bound thrombin, 27  28  lack of natural inhibitors against hirudin but present against heparin, 29  30  and high affinity for platelet thrombin receptor by r-hirudin, which can displace thrombin bound to platelet receptor.	bind
30001	3	7446	7	NULL	NULL	0	NULL	statement 2	NULL		displace	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_97_7_681_s_134	9495304	26  The superior antithrombotic efficacy of specific thrombin inhibition over heparin appears to be due to several mechanisms, including better inhibition of catalytically active clot-bound thrombin, 27  28  lack of natural inhibitors against hirudin but present against heparin, 29  30  and high affinity for platelet thrombin receptor by r-hirudin, which can displace thrombin bound to platelet receptor.	bind
30002	4	7446	7	10	NULL	0	NULL	thrombin		antithrombotic efficacy of;;inhibition of	is superior over					heparin					NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_7_681_s_134	9495304	26  The superior antithrombotic efficacy of specific thrombin inhibition over heparin appears to be due to several mechanisms, including better inhibition of catalytically active clot-bound thrombin, 27  28  lack of natural inhibitors against hirudin but present against heparin, 29  30  and high affinity for platelet thrombin receptor by r-hirudin, which can displace thrombin bound to platelet receptor.	bind
30003	5	7446	7	NULL	NULL	0	NULL	thrombin	NULL		bind	NULL				clot	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_7_681_s_134	9495304	26  The superior antithrombotic efficacy of specific thrombin inhibition over heparin appears to be due to several mechanisms, including better inhibition of catalytically active clot-bound thrombin, 27  28  lack of natural inhibitors against hirudin but present against heparin, 29  30  and high affinity for platelet thrombin receptor by r-hirudin, which can displace thrombin bound to platelet receptor.	bind
30004	6	7446	7	10	NULL	0	NULL	statement 4			is due to					statement 5		inhibition of;;catalytically active			NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_7_681_s_134	9495304	26  The superior antithrombotic efficacy of specific thrombin inhibition over heparin appears to be due to several mechanisms, including better inhibition of catalytically active clot-bound thrombin, 27  28  lack of natural inhibitors against hirudin but present against heparin, 29  30  and high affinity for platelet thrombin receptor by r-hirudin, which can displace thrombin bound to platelet receptor.	bind
30005	7	7446	7	NULL	NULL	0	NULL	hirudin	NULL		lacks	NULL				natural inhibitors	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_97_7_681_s_134	9495304	26  The superior antithrombotic efficacy of specific thrombin inhibition over heparin appears to be due to several mechanisms, including better inhibition of catalytically active clot-bound thrombin, 27  28  lack of natural inhibitors against hirudin but present against heparin, 29  30  and high affinity for platelet thrombin receptor by r-hirudin, which can displace thrombin bound to platelet receptor.	bind
30006	8	7446	7	NULL	NULL	0	NULL	statement 4	NULL		is due to	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_97_7_681_s_134	9495304	26  The superior antithrombotic efficacy of specific thrombin inhibition over heparin appears to be due to several mechanisms, including better inhibition of catalytically active clot-bound thrombin, 27  28  lack of natural inhibitors against hirudin but present against heparin, 29  30  and high affinity for platelet thrombin receptor by r-hirudin, which can displace thrombin bound to platelet receptor.	bind
30007	9	7446	7	NULL	NULL	0	NULL	statement 4	NULL		is due to	NULL				heparin	NULL	natural inhibitors against			NULL		0	NULL	NULL	NULL	gw60_circulation_97_7_681_s_134	9495304	26  The superior antithrombotic efficacy of specific thrombin inhibition over heparin appears to be due to several mechanisms, including better inhibition of catalytically active clot-bound thrombin, 27  28  lack of natural inhibitors against hirudin but present against heparin, 29  30  and high affinity for platelet thrombin receptor by r-hirudin, which can displace thrombin bound to platelet receptor.	bind
30008	10	7446	7	NULL	NULL	0	NULL	statement 4	NULL		is due to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_97_7_681_s_134	9495304	26  The superior antithrombotic efficacy of specific thrombin inhibition over heparin appears to be due to several mechanisms, including better inhibition of catalytically active clot-bound thrombin, 27  28  lack of natural inhibitors against hirudin but present against heparin, 29  30  and high affinity for platelet thrombin receptor by r-hirudin, which can displace thrombin bound to platelet receptor.	bind
28040	1	7447	5	13	NULL	NULL	NULL	anti-apo(a) antibody	GP		bind					THP-1 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2036_s_146	9351369	26  The y axis represents the amount of anti-apo(a) antibody bound to THP-1 cells or fibrin.	bind
28041	2	7447	5	13	NULL	NULL	NULL	anti-apo(a) antibody	GP		bind					fibrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2036_s_146	9351369	26  The y axis represents the amount of anti-apo(a) antibody bound to THP-1 cells or fibrin.	bind
30009	1	7447	7	NULL	NULL	0	NULL	anti-apo(a) antibody	NULL		bind	NULL				THP-1 cells	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2036_s_146	9351369	26  The y axis represents the amount of anti-apo(a) antibody bound to THP-1 cells or fibrin.	bind
30010	2	7447	7	NULL	NULL	0	NULL	anti-apo(a) antibody	NULL		bind	NULL				fibrin	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2036_s_146	9351369	26  The y axis represents the amount of anti-apo(a) antibody bound to THP-1 cells or fibrin.	bind
28042	1	7448	5	13	NULL	NULL	NULL	TIMP-3	GP		is secreted from					locally infected cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_3_296_s_168	10645926	26  TIMP-3 secreted from locally infected cells therefore binds tightly to the ECM surrounding cells at the luminal surface and in the upper media, but not substantially within the ECM of distant sites.	bind
28043	2	7448	5	13	NULL	NULL	NULL	statement 1	GP		bind					ECM surrounding cells	Cell				NULL	luminal surface, upper media	NULL	NULL	NULL	NULL	gw60_circulation_101_3_296_s_168	10645926	26  TIMP-3 secreted from locally infected cells therefore binds tightly to the ECM surrounding cells at the luminal surface and in the upper media, but not substantially within the ECM of distant sites.	bind
28044	3	7448	5	13	NULL	NULL	NULL	statement 1	GP		does not bind		substantially			ECM	CellComponent	distant sites			NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_3_296_s_168	10645926	26  TIMP-3 secreted from locally infected cells therefore binds tightly to the ECM surrounding cells at the luminal surface and in the upper media, but not substantially within the ECM of distant sites.	bind
30012	1	7448	7	NULL	NULL	0	NULL	TIMP-3	NULL		is secreted from	NULL				locally infected cells	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_101_3_296_s_168	10645926	26  TIMP-3 secreted from locally infected cells therefore binds tightly to the ECM surrounding cells at the luminal surface and in the upper media, but not substantially within the ECM of distant sites.	bind
30013	2	7448	7	10	NULL	0	NULL	TIMP-3			binds		tightly			ECM surrounding cells					NULL	luminal surface, upper media	NULL	NULL	NULL	NULL	gw60_circulation_101_3_296_s_168	10645926	26  TIMP-3 secreted from locally infected cells therefore binds tightly to the ECM surrounding cells at the luminal surface and in the upper media, but not substantially within the ECM of distant sites.	bind
30016	5	7448	7	10	NULL	0	NULL	TIMP-3			does not bind					ECM		distant site			NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_3_296_s_168	10645926	26  TIMP-3 secreted from locally infected cells therefore binds tightly to the ECM surrounding cells at the luminal surface and in the upper media, but not substantially within the ECM of distant sites.	bind
28045	1	7449	5	13	NULL	NULL	NULL	factor VIIa	GP		bind					tissue factor	GP				NULL	rabbit atherosclerotic model	NULL	NULL	NULL	NULL	gw60_circulation_94_12_3098_s_117	8989115	26 27  Blockage of factor VIIa binding to tissue factor as well as the use of recombinant tissue factor pathway inhibitor reduced angiographic restenosis and decreased neointimal hyperplasia in the rabbit atherosclerotic model.	bind
28046	2	7449	5	13	NULL	NULL	NULL	statement 1	Process	blockage of	reduces					angiographic restenosis	MedicalFinding				NULL	in  rabbit atherosclerotic model	NULL	NULL	NULL	NULL	gw60_circulation_94_12_3098_s_117	8989115	26 27  Blockage of factor VIIa binding to tissue factor as well as the use of recombinant tissue factor pathway inhibitor reduced angiographic restenosis and decreased neointimal hyperplasia in the rabbit atherosclerotic model.	bind
28047	3	7449	5	13	NULL	NULL	NULL	statement 1	Process	blockage of	decrease					hyperplasia	MedicalFinding	neointimal			NULL	in  rabbit atherosclerotic model	NULL	NULL	NULL	NULL	gw60_circulation_94_12_3098_s_117	8989115	26 27  Blockage of factor VIIa binding to tissue factor as well as the use of recombinant tissue factor pathway inhibitor reduced angiographic restenosis and decreased neointimal hyperplasia in the rabbit atherosclerotic model.	bind
28048	4	7449	5	13	NULL	NULL	NULL	tissue factor pathway inhibitor	GP	recombinant	reduces					angiographic restenosis	MedicalFinding				NULL	in  rabbit atherosclerotic model	NULL	NULL	NULL	NULL	gw60_circulation_94_12_3098_s_117	8989115	26 27  Blockage of factor VIIa binding to tissue factor as well as the use of recombinant tissue factor pathway inhibitor reduced angiographic restenosis and decreased neointimal hyperplasia in the rabbit atherosclerotic model.	bind
28049	5	7449	5	13	NULL	NULL	NULL	tissue factor pathway inhibitor	GP	recombinant	decrease					hyperplasia	MedicalFinding	neointimal			NULL	in  rabbit atherosclerotic model	NULL	NULL	NULL	NULL	gw60_circulation_94_12_3098_s_117	8989115	26 27  Blockage of factor VIIa binding to tissue factor as well as the use of recombinant tissue factor pathway inhibitor reduced angiographic restenosis and decreased neointimal hyperplasia in the rabbit atherosclerotic model.	bind
30017	1	7449	7	10	NULL	0	NULL	factor VIIa			bind					tissue factor					NULL	rabbit atherosclerotic model	NULL	NULL	NULL	NULL	gw60_circulation_94_12_3098_s_117	8989115	26 27  Blockage of factor VIIa binding to tissue factor as well as the use of recombinant tissue factor pathway inhibitor reduced angiographic restenosis and decreased neointimal hyperplasia in the rabbit atherosclerotic model.	bind
30018	2	7449	7	10	NULL	0	NULL	tissue factor pathway inhibitor		recombinant	reduce					angiographic restenosis					NULL	rabbit atherosclerotic model	NULL	NULL	NULL	NULL	gw60_circulation_94_12_3098_s_117	8989115	26 27  Blockage of factor VIIa binding to tissue factor as well as the use of recombinant tissue factor pathway inhibitor reduced angiographic restenosis and decreased neointimal hyperplasia in the rabbit atherosclerotic model.	bind
30020	3	7449	7	NULL	NULL	0	NULL	tissue factor pathway inhibitor	NULL	recombinant	decrease	NULL				neointimal hyperplasia 	NULL				NULL	 rabbit atherosclerotic model	0	NULL	NULL	NULL	gw60_circulation_94_12_3098_s_117	8989115	26 27  Blockage of factor VIIa binding to tissue factor as well as the use of recombinant tissue factor pathway inhibitor reduced angiographic restenosis and decreased neointimal hyperplasia in the rabbit atherosclerotic model.	bind
30022	4	7449	7	10	NULL	0	NULL	statement 1		blockage of	reduce					angiographic restenosis					NULL	rabbit atherosclerotic model	NULL	NULL	NULL	NULL	gw60_circulation_94_12_3098_s_117	8989115	26 27  Blockage of factor VIIa binding to tissue factor as well as the use of recombinant tissue factor pathway inhibitor reduced angiographic restenosis and decreased neointimal hyperplasia in the rabbit atherosclerotic model.	bind
30023	5	7449	7	NULL	NULL	0	NULL	statement 1	NULL	blockage of	decrease	NULL				neointimal hyperplasia 	NULL				NULL	rabbit atherosclerotic model	0	NULL	NULL	NULL	gw60_circulation_94_12_3098_s_117	8989115	26 27  Blockage of factor VIIa binding to tissue factor as well as the use of recombinant tissue factor pathway inhibitor reduced angiographic restenosis and decreased neointimal hyperplasia in the rabbit atherosclerotic model.	bind
28050	1	7450	5	13	NULL	NULL	NULL	von Willebrand factor	GP		bind					platelet gpIb	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1331_s_143	9261264	26 27  Shear stress-induced von Willebrand factor binding to platelet gpIb has been found to initiate calcium influx 28 29  and activation of protein kinase C, 30  both of which are known to trigger platelet secretion.	bind
28051	2	7450	5	13	NULL	NULL	NULL	shear stress			induces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1331_s_143	9261264	26 27  Shear stress-induced von Willebrand factor binding to platelet gpIb has been found to initiate calcium influx 28 29  and activation of protein kinase C, 30  both of which are known to trigger platelet secretion.	bind
28052	3	7450	5	13	NULL	NULL	NULL	statement 2	Process		initiates					calcium influx	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1331_s_143	9261264	26 27  Shear stress-induced von Willebrand factor binding to platelet gpIb has been found to initiate calcium influx 28 29  and activation of protein kinase C, 30  both of which are known to trigger platelet secretion.	bind
28053	4	7450	5	13	NULL	NULL	NULL	statement 2	Process		activates					protein kinase C	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1331_s_143	9261264	26 27  Shear stress-induced von Willebrand factor binding to platelet gpIb has been found to initiate calcium influx 28 29  and activation of protein kinase C, 30  both of which are known to trigger platelet secretion.	bind
28054	5	7450	5	13	NULL	NULL	NULL	statement 3	Process		triggers					platelet	Cell	secretion of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1331_s_143	9261264	26 27  Shear stress-induced von Willebrand factor binding to platelet gpIb has been found to initiate calcium influx 28 29  and activation of protein kinase C, 30  both of which are known to trigger platelet secretion.	bind
28055	6	7450	5	13	NULL	NULL	NULL	statement 4	Process		triggers					platelet	Cell	secretion of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1331_s_143	9261264	26 27  Shear stress-induced von Willebrand factor binding to platelet gpIb has been found to initiate calcium influx 28 29  and activation of protein kinase C, 30  both of which are known to trigger platelet secretion.	bind
30024	1	7450	7	NULL	NULL	0	NULL	Shear stress	NULL		induce	NULL				von Willebrand factor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1331_s_143	9261264	26 27  Shear stress-induced von Willebrand factor binding to platelet gpIb has been found to initiate calcium influx 28 29  and activation of protein kinase C, 30  both of which are known to trigger platelet secretion.	bind
30025	2	7450	7	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL				platelet gpIb	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1331_s_143	9261264	26 27  Shear stress-induced von Willebrand factor binding to platelet gpIb has been found to initiate calcium influx 28 29  and activation of protein kinase C, 30  both of which are known to trigger platelet secretion.	bind
30026	3	7450	7	NULL	NULL	0	NULL	statement 2	NULL		initiate	NULL				calcium influx	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1331_s_143	9261264	26 27  Shear stress-induced von Willebrand factor binding to platelet gpIb has been found to initiate calcium influx 28 29  and activation of protein kinase C, 30  both of which are known to trigger platelet secretion.	bind
30027	4	7450	7	NULL	NULL	0	NULL	statement 2	NULL		activates	NULL				protein kinase C	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1331_s_143	9261264	26 27  Shear stress-induced von Willebrand factor binding to platelet gpIb has been found to initiate calcium influx 28 29  and activation of protein kinase C, 30  both of which are known to trigger platelet secretion.	bind
30028	5	7450	7	10	NULL	0	NULL	statement 3			trigger					platelet		secretion of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1331_s_143	9261264	26 27  Shear stress-induced von Willebrand factor binding to platelet gpIb has been found to initiate calcium influx 28 29  and activation of protein kinase C, 30  both of which are known to trigger platelet secretion.	bind
30029	6	7450	7	10	NULL	0	NULL	statement 4			trigger					platelet		secretion of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1331_s_143	9261264	26 27  Shear stress-induced von Willebrand factor binding to platelet gpIb has been found to initiate calcium influx 28 29  and activation of protein kinase C, 30  both of which are known to trigger platelet secretion.	bind
28056	1	7451	5	13	NULL	NULL	NULL	AT1-R antagonists	Chemical		increases					Ang II	GP	circulating levels of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_11_3954_s_247	9403620	26 27 28 29  Because circulating Ang II levels are increased by treatment with AT1-R antagonists 45  and Ang II preferentially binds to cardiac AT2-R, AT2-R - mediated actions are expected to be further activated under these pathological conditions.	bind
28057	2	7451	5	13	NULL	NULL	NULL	Ang II	GP		bind		preferentially			AT2-R	GP	cardiac			NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_11_3954_s_247	9403620	26 27 28 29  Because circulating Ang II levels are increased by treatment with AT1-R antagonists 45  and Ang II preferentially binds to cardiac AT2-R, AT2-R - mediated actions are expected to be further activated under these pathological conditions.	bind
30036	1	7451	7	NULL	NULL	0	NULL	AT1-R antagonists	NULL		increase	NULL				AngII	NULL	circulating levels of 			NULL		0	NULL	NULL	NULL	gw60_circulation_96_11_3954_s_247	9403620	26 27 28 29  Because circulating Ang II levels are increased by treatment with AT1-R antagonists 45  and Ang II preferentially binds to cardiac AT2-R, AT2-R - mediated actions are expected to be further activated under these pathological conditions.	bind
30037	2	7451	7	NULL	NULL	0	NULL	 Ang II 	NULL		binds	NULL	preferentially			AT2-R	NULL	cardiac			NULL		0	NULL	NULL	NULL	gw60_circulation_96_11_3954_s_247	9403620	26 27 28 29  Because circulating Ang II levels are increased by treatment with AT1-R antagonists 45  and Ang II preferentially binds to cardiac AT2-R, AT2-R - mediated actions are expected to be further activated under these pathological conditions.	bind
28058	1	7452	5	13	NULL	NULL	NULL	E1A	GP		bind					pocket protein	GP				NULL	in cardiac muscle	NULL	NULL	NULL	NULL	gw60_circulationres_85_4_319_s_33	10455060	26 29 30  Forced expression of E2F-1, the prototype for E2F proteins that are the best understood endogenous occupants of the "`pocket,"` was sufficient by itself to reproduce the effect of pocket protein binding by E1A on G1 exit in cardiac muscle, 26  27  a finding also seen in other cell backgrounds.	bind
28059	3	7452	5	13	NULL	NULL	NULL	E2F-1	GP		reproduce		sufficiently			statement 1	Process	effect of 			NULL	in cardiac muscle	NULL	NULL	NULL	NULL	gw60_circulationres_85_4_319_s_33	10455060	26 29 30  Forced expression of E2F-1, the prototype for E2F proteins that are the best understood endogenous occupants of the "`pocket,"` was sufficient by itself to reproduce the effect of pocket protein binding by E1A on G1 exit in cardiac muscle, 26  27  a finding also seen in other cell backgrounds.	bind
28060	2	7452	5	13	NULL	NULL	NULL	statement 1	Process		occurs in					G1 exit	Process				NULL	in cardiac muscle	NULL	NULL	NULL	NULL	gw60_circulationres_85_4_319_s_33	10455060	26 29 30  Forced expression of E2F-1, the prototype for E2F proteins that are the best understood endogenous occupants of the "`pocket,"` was sufficient by itself to reproduce the effect of pocket protein binding by E1A on G1 exit in cardiac muscle, 26  27  a finding also seen in other cell backgrounds.	bind
28061	4	7452	5	13	NULL	NULL	NULL	E2F-1	GP		is a prototype for					E2F proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_4_319_s_33	10455060	26 29 30  Forced expression of E2F-1, the prototype for E2F proteins that are the best understood endogenous occupants of the "`pocket,"` was sufficient by itself to reproduce the effect of pocket protein binding by E1A on G1 exit in cardiac muscle, 26  27  a finding also seen in other cell backgrounds.	bind
28062	5	7452	5	13	NULL	NULL	NULL	E2F proteins	GP		occupants of		endogenous			pocket	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_4_319_s_33	10455060	26 29 30  Forced expression of E2F-1, the prototype for E2F proteins that are the best understood endogenous occupants of the "`pocket,"` was sufficient by itself to reproduce the effect of pocket protein binding by E1A on G1 exit in cardiac muscle, 26  27  a finding also seen in other cell backgrounds.	bind
30067	1	7452	7	NULL	NULL	0	NULL	E1A	NULL		bind	NULL				pocket proteins	NULL				NULL	cardiac muscle	NULL	NULL	NULL	NULL	gw60_circulationres_85_4_319_s_33	10455060	26 29 30  Forced expression of E2F-1, the prototype for E2F proteins that are the best understood endogenous occupants of the "`pocket,"` was sufficient by itself to reproduce the effect of pocket protein binding by E1A on G1 exit in cardiac muscle, 26  27  a finding also seen in other cell backgrounds.	bind
30068	2	7452	7	NULL	NULL	0	NULL	statement 1	NULL		occurs upon	NULL				G1 	NULL	exit of			NULL	cardiac muscle	NULL	NULL	NULL	NULL	gw60_circulationres_85_4_319_s_33	10455060	26 29 30  Forced expression of E2F-1, the prototype for E2F proteins that are the best understood endogenous occupants of the "`pocket,"` was sufficient by itself to reproduce the effect of pocket protein binding by E1A on G1 exit in cardiac muscle, 26  27  a finding also seen in other cell backgrounds.	bind
30069	3	7452	7	NULL	NULL	0	NULL	E2F-1	NULL		is a prototype for	NULL				E2F proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_85_4_319_s_33	10455060	26 29 30  Forced expression of E2F-1, the prototype for E2F proteins that are the best understood endogenous occupants of the "`pocket,"` was sufficient by itself to reproduce the effect of pocket protein binding by E1A on G1 exit in cardiac muscle, 26  27  a finding also seen in other cell backgrounds.	bind
30070	4	7452	7	10	NULL	0	NULL	E2F proteins			occupants of		endogenous			pocket					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_4_319_s_33	10455060	26 29 30  Forced expression of E2F-1, the prototype for E2F proteins that are the best understood endogenous occupants of the "`pocket,"` was sufficient by itself to reproduce the effect of pocket protein binding by E1A on G1 exit in cardiac muscle, 26  27  a finding also seen in other cell backgrounds.	bind
30475	5	7452	7	NULL	NULL	0	NULL	E2F-1	NULL		bind	NULL				pocket proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_85_4_319_s_33	10455060	26 29 30  Forced expression of E2F-1, the prototype for E2F proteins that are the best understood endogenous occupants of the "`pocket,"` was sufficient by itself to reproduce the effect of pocket protein binding by E1A on G1 exit in cardiac muscle, 26  27  a finding also seen in other cell backgrounds.	bind
28063	1	7453	5	13	NULL	NULL	NULL	HSP90	GP		bind					eNOS	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_959_s_26	16627819	26 Although binding of HSP90 to eNOS in response to VEGF and fluid shear stress increases eNOS activity by facilitating CaM-induced displacement of caveolin-1 from endogenous eNOS, 27 it remains unclear whether there is any change in caveolin-1 interaction with the PM eNOS versus the Golgi-PM in response to agonists.	bind
28064	2	7453	5	13	NULL	NULL	NULL	statement 1	Process		occurs in response to					VEGF	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_959_s_26	16627819	26 Although binding of HSP90 to eNOS in response to VEGF and fluid shear stress increases eNOS activity by facilitating CaM-induced displacement of caveolin-1 from endogenous eNOS, 27 it remains unclear whether there is any change in caveolin-1 interaction with the PM eNOS versus the Golgi-PM in response to agonists.	bind
28065	3	7453	5	13	NULL	NULL	NULL	statement 1	Process		occurs in response to					fluid shear stress					NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_959_s_26	16627819	26 Although binding of HSP90 to eNOS in response to VEGF and fluid shear stress increases eNOS activity by facilitating CaM-induced displacement of caveolin-1 from endogenous eNOS, 27 it remains unclear whether there is any change in caveolin-1 interaction with the PM eNOS versus the Golgi-PM in response to agonists.	bind
28066	4	7453	5	13	NULL	NULL	NULL	statement 2	Process		increases					eNOS	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_959_s_26	16627819	26 Although binding of HSP90 to eNOS in response to VEGF and fluid shear stress increases eNOS activity by facilitating CaM-induced displacement of caveolin-1 from endogenous eNOS, 27 it remains unclear whether there is any change in caveolin-1 interaction with the PM eNOS versus the Golgi-PM in response to agonists.	bind
28067	5	7453	5	13	NULL	NULL	NULL	statement 3	Process		increases					eNOS	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_959_s_26	16627819	26 Although binding of HSP90 to eNOS in response to VEGF and fluid shear stress increases eNOS activity by facilitating CaM-induced displacement of caveolin-1 from endogenous eNOS, 27 it remains unclear whether there is any change in caveolin-1 interaction with the PM eNOS versus the Golgi-PM in response to agonists.	bind
28068	6	7453	5	13	NULL	NULL	NULL	caveolin-1	GP		is displaced from					eNOS	GP	endogenous			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_959_s_26	16627819	26 Although binding of HSP90 to eNOS in response to VEGF and fluid shear stress increases eNOS activity by facilitating CaM-induced displacement of caveolin-1 from endogenous eNOS, 27 it remains unclear whether there is any change in caveolin-1 interaction with the PM eNOS versus the Golgi-PM in response to agonists.	bind
28069	7	7453	5	13	NULL	NULL	NULL	CaM	GP		induces					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_959_s_26	16627819	26 Although binding of HSP90 to eNOS in response to VEGF and fluid shear stress increases eNOS activity by facilitating CaM-induced displacement of caveolin-1 from endogenous eNOS, 27 it remains unclear whether there is any change in caveolin-1 interaction with the PM eNOS versus the Golgi-PM in response to agonists.	bind
28070	8	7453	5	13	NULL	NULL	NULL	statement 4	Process		occurs by					statement 7	Process	facilitating			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_959_s_26	16627819	26 Although binding of HSP90 to eNOS in response to VEGF and fluid shear stress increases eNOS activity by facilitating CaM-induced displacement of caveolin-1 from endogenous eNOS, 27 it remains unclear whether there is any change in caveolin-1 interaction with the PM eNOS versus the Golgi-PM in response to agonists.	bind
28071	9	7453	5	13	NULL	NULL	NULL	statement 5	Process		occurs by					statement 7	Process	facilitating			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_959_s_26	16627819	26 Although binding of HSP90 to eNOS in response to VEGF and fluid shear stress increases eNOS activity by facilitating CaM-induced displacement of caveolin-1 from endogenous eNOS, 27 it remains unclear whether there is any change in caveolin-1 interaction with the PM eNOS versus the Golgi-PM in response to agonists.	bind
28072	10	7453	5	13	NULL	NULL	NULL	caveolin-1	GP		interacts with					eNOS	GP	PM			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_959_s_26	16627819	26 Although binding of HSP90 to eNOS in response to VEGF and fluid shear stress increases eNOS activity by facilitating CaM-induced displacement of caveolin-1 from endogenous eNOS, 27 it remains unclear whether there is any change in caveolin-1 interaction with the PM eNOS versus the Golgi-PM in response to agonists.	bind
28073	11	7453	5	13	NULL	NULL	NULL	caveolin-1	GP		interacts with					Golgi-PM	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_959_s_26	16627819	26 Although binding of HSP90 to eNOS in response to VEGF and fluid shear stress increases eNOS activity by facilitating CaM-induced displacement of caveolin-1 from endogenous eNOS, 27 it remains unclear whether there is any change in caveolin-1 interaction with the PM eNOS versus the Golgi-PM in response to agonists.	bind
30039	1	7453	7	NULL	NULL	0	NULL	HSP90	NULL		bind	NULL				eNOS	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_959_s_26	16627819	26 Although binding of HSP90 to eNOS in response to VEGF and fluid shear stress increases eNOS activity by facilitating CaM-induced displacement of caveolin-1 from endogenous eNOS, 27 it remains unclear whether there is any change in caveolin-1 interaction with the PM eNOS versus the Golgi-PM in response to agonists.	bind
30040	2	7453	7	NULL	NULL	0	NULL	statement 1	NULL		in response to	NULL				VEGF	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_959_s_26	16627819	26 Although binding of HSP90 to eNOS in response to VEGF and fluid shear stress increases eNOS activity by facilitating CaM-induced displacement of caveolin-1 from endogenous eNOS, 27 it remains unclear whether there is any change in caveolin-1 interaction with the PM eNOS versus the Golgi-PM in response to agonists.	bind
30041	5	7453	7	NULL	NULL	0	NULL	statement 1			increase					eNOS		activity of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_959_s_26	16627819	26 Although binding of HSP90 to eNOS in response to VEGF and fluid shear stress increases eNOS activity by facilitating CaM-induced displacement of caveolin-1 from endogenous eNOS, 27 it remains unclear whether there is any change in caveolin-1 interaction with the PM eNOS versus the Golgi-PM in response to agonists.	bind
30042	7	7453	7	10	NULL	0	NULL	CaM			induce					statement 6					NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_959_s_26	16627819	26 Although binding of HSP90 to eNOS in response to VEGF and fluid shear stress increases eNOS activity by facilitating CaM-induced displacement of caveolin-1 from endogenous eNOS, 27 it remains unclear whether there is any change in caveolin-1 interaction with the PM eNOS versus the Golgi-PM in response to agonists.	bind
30043	6	7453	7	NULL	NULL	0	NULL	caveolin-1			displaced from					eNOS		endogenous			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_959_s_26	16627819	26 Although binding of HSP90 to eNOS in response to VEGF and fluid shear stress increases eNOS activity by facilitating CaM-induced displacement of caveolin-1 from endogenous eNOS, 27 it remains unclear whether there is any change in caveolin-1 interaction with the PM eNOS versus the Golgi-PM in response to agonists.	bind
30044	8	7453	7	10	NULL	0	NULL	statement 5			occur by					statement 7		facilitating			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_959_s_26	16627819	26 Although binding of HSP90 to eNOS in response to VEGF and fluid shear stress increases eNOS activity by facilitating CaM-induced displacement of caveolin-1 from endogenous eNOS, 27 it remains unclear whether there is any change in caveolin-1 interaction with the PM eNOS versus the Golgi-PM in response to agonists.	bind
30045	9	7453	7	NULL	NULL	0	NULL	caveolin-1 			interacts with					eNOS		PM			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_959_s_26	16627819	26 Although binding of HSP90 to eNOS in response to VEGF and fluid shear stress increases eNOS activity by facilitating CaM-induced displacement of caveolin-1 from endogenous eNOS, 27 it remains unclear whether there is any change in caveolin-1 interaction with the PM eNOS versus the Golgi-PM in response to agonists.	bind
30046	10	7453	7	10	NULL	0	NULL	caveolin-1			interacts with					Golgi-PM					NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_959_s_26	16627819	26 Although binding of HSP90 to eNOS in response to VEGF and fluid shear stress increases eNOS activity by facilitating CaM-induced displacement of caveolin-1 from endogenous eNOS, 27 it remains unclear whether there is any change in caveolin-1 interaction with the PM eNOS versus the Golgi-PM in response to agonists.	bind
54676	3	7453	7	NULL	NULL	0	NULL	statement 1			in response to					fluid shear stress					NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_959_s_26	16627819	26 Although binding of HSP90 to eNOS in response to VEGF and fluid shear stress increases eNOS activity by facilitating CaM-induced displacement of caveolin-1 from endogenous eNOS, 27 it remains unclear whether there is any change in caveolin-1 interaction with the PM eNOS versus the Golgi-PM in response to agonists.	bind
54677	4	7453	7	NULL	NULL	0	NULL	statement 2			occur along with					statement 3					NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_5_959_s_26	16627819	26 Although binding of HSP90 to eNOS in response to VEGF and fluid shear stress increases eNOS activity by facilitating CaM-induced displacement of caveolin-1 from endogenous eNOS, 27 it remains unclear whether there is any change in caveolin-1 interaction with the PM eNOS versus the Golgi-PM in response to agonists.	bind
28074	1	7454	5	13	NULL	NULL	NULL	SUR2B	GP		bind			NBD2		ADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_5_554_s_202	11909819	26 Because it was reported that NBD2 of SUR2B exhibits higherR binding capability to ADP than that of SUR2A 27 and because the primary function of Walker-A loop is to bind nucleotides, it seems likely that the difference between SUR2A and SUR2B in the binding property of ADP to their NBD2 may be one of the most possible candidates.	bind
28075	2	7454	5	13	NULL	NULL	NULL	SUR2A	GP		bind			NBD2		ADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_5_554_s_202	11909819	26 Because it was reported that NBD2 of SUR2B exhibits higherR binding capability to ADP than that of SUR2A 27 and because the primary function of Walker-A loop is to bind nucleotides, it seems likely that the difference between SUR2A and SUR2B in the binding property of ADP to their NBD2 may be one of the most possible candidates.	bind
28076	3	7454	5	13	NULL	NULL	NULL	statement 1	GP		higher binding capability than					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_5_554_s_202	11909819	26 Because it was reported that NBD2 of SUR2B exhibits higherR binding capability to ADP than that of SUR2A 27 and because the primary function of Walker-A loop is to bind nucleotides, it seems likely that the difference between SUR2A and SUR2B in the binding property of ADP to their NBD2 may be one of the most possible candidates.	bind
28077	4	7454	5	13	NULL	NULL	NULL				bind			Walker-A loop		nucleotides	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_5_554_s_202	11909819	26 Because it was reported that NBD2 of SUR2B exhibits higherR binding capability to ADP than that of SUR2A 27 and because the primary function of Walker-A loop is to bind nucleotides, it seems likely that the difference between SUR2A and SUR2B in the binding property of ADP to their NBD2 may be one of the most possible candidates.	bind
30047	1	7454	7	NULL	NULL	0	NULL	SUR2B	NULL		bind	NULL		NBD2		ADP	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_5_554_s_202	11909819	26 Because it was reported that NBD2 of SUR2B exhibits higherR binding capability to ADP than that of SUR2A 27 and because the primary function of Walker-A loop is to bind nucleotides, it seems likely that the difference between SUR2A and SUR2B in the binding property of ADP to their NBD2 may be one of the most possible candidates.	bind
30048	2	7454	7	10	NULL	0	NULL	SUR2A	NULL		bind	NULL		NBD2		ADP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_5_554_s_202	11909819	26 Because it was reported that NBD2 of SUR2B exhibits higherR binding capability to ADP than that of SUR2A 27 and because the primary function of Walker-A loop is to bind nucleotides, it seems likely that the difference between SUR2A and SUR2B in the binding property of ADP to their NBD2 may be one of the most possible candidates.	bind
30049	3	7454	7	NULL	NULL	0	NULL	statement 1	NULL		higher affinity than	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_5_554_s_202	11909819	26 Because it was reported that NBD2 of SUR2B exhibits higherR binding capability to ADP than that of SUR2A 27 and because the primary function of Walker-A loop is to bind nucleotides, it seems likely that the difference between SUR2A and SUR2B in the binding property of ADP to their NBD2 may be one of the most possible candidates.	bind
30050	4	7454	7	NULL	NULL	0	NULL		NULL		bind	NULL		Walker-A loop		nucleotides	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_5_554_s_202	11909819	26 Because it was reported that NBD2 of SUR2B exhibits higherR binding capability to ADP than that of SUR2A 27 and because the primary function of Walker-A loop is to bind nucleotides, it seems likely that the difference between SUR2A and SUR2B in the binding property of ADP to their NBD2 may be one of the most possible candidates.	bind
28078	1	7455	5	13	NULL	NULL	NULL	procaspase-9	GP		bind					Apaf-1	GP				NULL	in cytosol	NULL	NULL	NULL	NULL	gw60_circulationres_89_3_279_s_108	11485979	26 By immunoprecipitation of myocyte proteins with Apaf-1 antibody and subsequent exposure of the immunoprecipitated proteins to anti - procaspase-9 and Western blot, the fraction of procaspase-9 bound to Apaf-1 was detected in the cytosol ( Figure 3D).	bind
30051	1	7455	7	NULL	NULL	0	NULL	procaspase-9	NULL		bind	NULL				Apaf-1	NULL				NULL	cytosol	0	NULL	NULL	NULL	gw60_circulationres_89_3_279_s_108	11485979	26 By immunoprecipitation of myocyte proteins with Apaf-1 antibody and subsequent exposure of the immunoprecipitated proteins to anti - procaspase-9 and Western blot, the fraction of procaspase-9 bound to Apaf-1 was detected in the cytosol ( Figure 3D).	bind
28079	1	7456	5	13	NULL	NULL	NULL	ricin lectin	GP	rhodamine-labeled	bind		weakly			luminal surface	OrganismPart	endothelial			NULL	in untreated vessels	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2108_s_108	15345507	26 In untreated vessels, rhodamine-labeled ricin lectin binding to the endothelial luminal surface was weak and uniform in both genotypes (data not shown).	bind
30052	1	7456	7	10	NULL	0	NULL	ricin lectin	NULL	rhodamine-labeled	bind	NULL	weakly			 luminal surface	NULL	endothelial			NULL	untreated vessels	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2108_s_108	15345507	26 In untreated vessels, rhodamine-labeled ricin lectin binding to the endothelial luminal surface was weak and uniform in both genotypes (data not shown).	bind
28080	1	7457	5	13	NULL	NULL	NULL	C4BPbeta+ isoform molecules	GP		bind					PS	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_508_s_106	12615682	26 In vivo, all C4BPbeta+ isoform molecules circulate bound to PS.	bind
30053	1	7457	7	NULL	NULL	0	NULL	C4BPbeta+ isoform molecules	NULL		bind	NULL				PS	NULL				NULL	in vivo	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_508_s_106	12615682	26 In vivo, all C4BPbeta+ isoform molecules circulate bound to PS.	bind
28081	1	7458	5	13	NULL	NULL	NULL	KIAA1437	GP		bind					k-ras	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_19_2467_s_157	12742993	26 KIAA1437 binds k-ras, where k-ras - deficient mice develop a thin ventricular wall and die until term.	bind
28082	2	7458	5	13	NULL	NULL	NULL	k-ras	GP	mice deficient in	develop					ventricular wall	OrganismPart	thin			NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_19_2467_s_157	12742993	26 KIAA1437 binds k-ras, where k-ras - deficient mice develop a thin ventricular wall and die until term.	bind
30055	1	7458	7	NULL	NULL	0	NULL	KIAA1437	NULL		binds	NULL				k-ras	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_107_19_2467_s_157	12742993	26 KIAA1437 binds k-ras, where k-ras - deficient mice develop a thin ventricular wall and die until term.	bind
30056	2	7458	7	10	NULL	0	NULL	k-ras - 		mice deficient in	develop					ventricular wall		thin			NULL		NULL	NULL	NULL	NULL	gw60_circulation_107_19_2467_s_157	12742993	26 KIAA1437 binds k-ras, where k-ras - deficient mice develop a thin ventricular wall and die until term.	bind
29897	1	7459	5	13	NULL	NULL	NULL	TRL	GP		bind					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_5_805_s_115	12006394	26 The E2 allele is also known to demonstrate impaired TRL binding by the LDL receptor 27 and more recently, has been shown to be associated with impaired lipoprotein lipase - mediated lipolysis of TRLs. 28 The greatest increase in LDL cholesterol associated with the L162V polymorphism ( Figure 1) was seen in carriers of the E2 allele and the smallest in those with the E4 allele.	bind
29900	2	7459	5	13	NULL	NULL	NULL	E2 allele	GP		impairs					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_5_805_s_115	12006394	26 The E2 allele is also known to demonstrate impaired TRL binding by the LDL receptor 27 and more recently, has been shown to be associated with impaired lipoprotein lipase - mediated lipolysis of TRLs. 28 The greatest increase in LDL cholesterol associated with the L162V polymorphism ( Figure 1) was seen in carriers of the E2 allele and the smallest in those with the E4 allele.	bind
29903	3	7459	5	13	NULL	NULL	NULL	lipoprotein lipase	GP		mediate					TRLs	GP	lipolysis of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_5_805_s_115	12006394	26 The E2 allele is also known to demonstrate impaired TRL binding by the LDL receptor 27 and more recently, has been shown to be associated with impaired lipoprotein lipase - mediated lipolysis of TRLs. 28 The greatest increase in LDL cholesterol associated with the L162V polymorphism ( Figure 1) was seen in carriers of the E2 allele and the smallest in those with the E4 allele.	bind
29904	4	7459	5	13	NULL	NULL	NULL	E2 allele	GP		is associtaed with					statement 3	Process	impaired			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_5_805_s_115	12006394	26 The E2 allele is also known to demonstrate impaired TRL binding by the LDL receptor 27 and more recently, has been shown to be associated with impaired lipoprotein lipase - mediated lipolysis of TRLs. 28 The greatest increase in LDL cholesterol associated with the L162V polymorphism ( Figure 1) was seen in carriers of the E2 allele and the smallest in those with the E4 allele.	bind
29932	5	7459	5	13	NULL	NULL	NULL	LDL cholesterol	Chemical	increase in	is associtaed with					L162V polymorphism	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_5_805_s_115	12006394	26 The E2 allele is also known to demonstrate impaired TRL binding by the LDL receptor 27 and more recently, has been shown to be associated with impaired lipoprotein lipase - mediated lipolysis of TRLs. 28 The greatest increase in LDL cholesterol associated with the L162V polymorphism ( Figure 1) was seen in carriers of the E2 allele and the smallest in those with the E4 allele.	bind
29933	6	7459	5	13	NULL	NULL	NULL	statement 5	Process		is seen in					E2 allele	GP	carriers of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_5_805_s_115	12006394	26 The E2 allele is also known to demonstrate impaired TRL binding by the LDL receptor 27 and more recently, has been shown to be associated with impaired lipoprotein lipase - mediated lipolysis of TRLs. 28 The greatest increase in LDL cholesterol associated with the L162V polymorphism ( Figure 1) was seen in carriers of the E2 allele and the smallest in those with the E4 allele.	bind
29934	7	7459	5	13	NULL	NULL	NULL	statement 5	Process		is seen in					E4 allele	GP	carriers of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_5_805_s_115	12006394	26 The E2 allele is also known to demonstrate impaired TRL binding by the LDL receptor 27 and more recently, has been shown to be associated with impaired lipoprotein lipase - mediated lipolysis of TRLs. 28 The greatest increase in LDL cholesterol associated with the L162V polymorphism ( Figure 1) was seen in carriers of the E2 allele and the smallest in those with the E4 allele.	bind
30058	1	7459	7	NULL	NULL	0	NULL	LDL receptor	NULL		bind	NULL				TRL	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_5_805_s_115	12006394	26 The E2 allele is also known to demonstrate impaired TRL binding by the LDL receptor 27 and more recently, has been shown to be associated with impaired lipoprotein lipase - mediated lipolysis of TRLs. 28 The greatest increase in LDL cholesterol associated with the L162V polymorphism ( Figure 1) was seen in carriers of the E2 allele and the smallest in those with the E4 allele.	bind
30059	2	7459	7	NULL	NULL	0	NULL	E2 allele	NULL		impairs	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_5_805_s_115	12006394	26 The E2 allele is also known to demonstrate impaired TRL binding by the LDL receptor 27 and more recently, has been shown to be associated with impaired lipoprotein lipase - mediated lipolysis of TRLs. 28 The greatest increase in LDL cholesterol associated with the L162V polymorphism ( Figure 1) was seen in carriers of the E2 allele and the smallest in those with the E4 allele.	bind
30060	3	7459	7	NULL	NULL	0	NULL	lipoprotein lipase	NULL		mediates	NULL				TRLs	NULL	lipolysis of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_5_805_s_115	12006394	26 The E2 allele is also known to demonstrate impaired TRL binding by the LDL receptor 27 and more recently, has been shown to be associated with impaired lipoprotein lipase - mediated lipolysis of TRLs. 28 The greatest increase in LDL cholesterol associated with the L162V polymorphism ( Figure 1) was seen in carriers of the E2 allele and the smallest in those with the E4 allele.	bind
30476	4	7459	7	NULL	NULL	0	NULL	E2 allele	NULL		impairs	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_5_805_s_115	12006394	26 The E2 allele is also known to demonstrate impaired TRL binding by the LDL receptor 27 and more recently, has been shown to be associated with impaired lipoprotein lipase - mediated lipolysis of TRLs. 28 The greatest increase in LDL cholesterol associated with the L162V polymorphism ( Figure 1) was seen in carriers of the E2 allele and the smallest in those with the E4 allele.	bind
30477	5	7459	7	NULL	NULL	0	NULL	LDL cholesterol 	NULL	increase in	is associated with	NULL				polymorph	NULL		L162V		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_5_805_s_115	12006394	26 The E2 allele is also known to demonstrate impaired TRL binding by the LDL receptor 27 and more recently, has been shown to be associated with impaired lipoprotein lipase - mediated lipolysis of TRLs. 28 The greatest increase in LDL cholesterol associated with the L162V polymorphism ( Figure 1) was seen in carriers of the E2 allele and the smallest in those with the E4 allele.	bind
30478	6	7459	7	10	NULL	0	NULL	statement 5			is seen in 					E2 allele		carriers of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_5_805_s_115	12006394	26 The E2 allele is also known to demonstrate impaired TRL binding by the LDL receptor 27 and more recently, has been shown to be associated with impaired lipoprotein lipase - mediated lipolysis of TRLs. 28 The greatest increase in LDL cholesterol associated with the L162V polymorphism ( Figure 1) was seen in carriers of the E2 allele and the smallest in those with the E4 allele.	bind
30479	7	7459	7	10	NULL	0	NULL	statement 5			is seen in 					E4 allele		carriers of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_5_805_s_115	12006394	26 The E2 allele is also known to demonstrate impaired TRL binding by the LDL receptor 27 and more recently, has been shown to be associated with impaired lipoprotein lipase - mediated lipolysis of TRLs. 28 The greatest increase in LDL cholesterol associated with the L162V polymorphism ( Figure 1) was seen in carriers of the E2 allele and the smallest in those with the E4 allele.	bind
30480	8	7459	7	NULL	NULL	0	NULL	statement 7	NULL	increase in	is less than	NULL				statement 6	NULL	increase in			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_5_805_s_115	12006394	26 The E2 allele is also known to demonstrate impaired TRL binding by the LDL receptor 27 and more recently, has been shown to be associated with impaired lipoprotein lipase - mediated lipolysis of TRLs. 28 The greatest increase in LDL cholesterol associated with the L162V polymorphism ( Figure 1) was seen in carriers of the E2 allele and the smallest in those with the E4 allele.	bind
30144	1	7460	5	13	NULL	NULL	NULL	MYPT1	GP		bind		strong			PP1c	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulationres_90_5_546_s_181	11909818	26 Thus, in vitro, the binding of MYPT1 and PP1c is relatively strong.	bind
30071	1	7460	7	NULL	NULL	0	NULL	MYPT1	NULL		bind	NULL	strongly			PP1c	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_circulationres_90_5_546_s_181	11909818	26 Thus, in vitro, the binding of MYPT1 and PP1c is relatively strong.	bind
28085	1	7461	5	13	NULL	NULL	NULL	VWF	GP		does not bind					rHPA-2a	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1302_s_117	12775575	26 Whereas no binding of VWF to either rHPA-2a or rHPA-2b could be observed in the absence of ristocetin (not shown), both dose dependently interacted with VWF in the presence of 1500 mug/mL ristocetin ( Figure 3A) with a Kd,app of, respectively, 0.69 plus-or-minus 0.06 and 0.67 plus-or-minus 0.03 nmol/L (mean plus-or-minus SE) ( P=0.80), showing no statistical difference in VWF interaction at this ristocetin concentration.	bind
28086	2	7461	5	13	NULL	NULL	NULL	VWF	GP		does not bind					rHPA-2b	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1302_s_117	12775575	26 Whereas no binding of VWF to either rHPA-2a or rHPA-2b could be observed in the absence of ristocetin (not shown), both dose dependently interacted with VWF in the presence of 1500 mug/mL ristocetin ( Figure 3A) with a Kd,app of, respectively, 0.69 plus-or-minus 0.06 and 0.67 plus-or-minus 0.03 nmol/L (mean plus-or-minus SE) ( P=0.80), showing no statistical difference in VWF interaction at this ristocetin concentration.	bind
28087	3	7461	5	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1302_s_117	12775575	26 Whereas no binding of VWF to either rHPA-2a or rHPA-2b could be observed in the absence of ristocetin (not shown), both dose dependently interacted with VWF in the presence of 1500 mug/mL ristocetin ( Figure 3A) with a Kd,app of, respectively, 0.69 plus-or-minus 0.06 and 0.67 plus-or-minus 0.03 nmol/L (mean plus-or-minus SE) ( P=0.80), showing no statistical difference in VWF interaction at this ristocetin concentration.	bind
28088	4	7461	5	13	NULL	NULL	NULL	statement 1	Process		in the absence of					ristocetin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1302_s_117	12775575	26 Whereas no binding of VWF to either rHPA-2a or rHPA-2b could be observed in the absence of ristocetin (not shown), both dose dependently interacted with VWF in the presence of 1500 mug/mL ristocetin ( Figure 3A) with a Kd,app of, respectively, 0.69 plus-or-minus 0.06 and 0.67 plus-or-minus 0.03 nmol/L (mean plus-or-minus SE) ( P=0.80), showing no statistical difference in VWF interaction at this ristocetin concentration.	bind
28089	5	7461	5	13	NULL	NULL	NULL	statement 2	Process		in the absence of					ristocetin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1302_s_117	12775575	26 Whereas no binding of VWF to either rHPA-2a or rHPA-2b could be observed in the absence of ristocetin (not shown), both dose dependently interacted with VWF in the presence of 1500 mug/mL ristocetin ( Figure 3A) with a Kd,app of, respectively, 0.69 plus-or-minus 0.06 and 0.67 plus-or-minus 0.03 nmol/L (mean plus-or-minus SE) ( P=0.80), showing no statistical difference in VWF interaction at this ristocetin concentration.	bind
28090	6	7461	5	13	NULL	NULL	NULL	rHPA-2a	GP		interacts with		dose dependently			VWF	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1302_s_117	12775575	26 Whereas no binding of VWF to either rHPA-2a or rHPA-2b could be observed in the absence of ristocetin (not shown), both dose dependently interacted with VWF in the presence of 1500 mug/mL ristocetin ( Figure 3A) with a Kd,app of, respectively, 0.69 plus-or-minus 0.06 and 0.67 plus-or-minus 0.03 nmol/L (mean plus-or-minus SE) ( P=0.80), showing no statistical difference in VWF interaction at this ristocetin concentration.	bind
28091	7	7461	5	13	NULL	NULL	NULL	statement 6	Process		in the presence of					ristocetin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1302_s_117	12775575	26 Whereas no binding of VWF to either rHPA-2a or rHPA-2b could be observed in the absence of ristocetin (not shown), both dose dependently interacted with VWF in the presence of 1500 mug/mL ristocetin ( Figure 3A) with a Kd,app of, respectively, 0.69 plus-or-minus 0.06 and 0.67 plus-or-minus 0.03 nmol/L (mean plus-or-minus SE) ( P=0.80), showing no statistical difference in VWF interaction at this ristocetin concentration.	bind
28092	8	7461	5	13	NULL	NULL	NULL	rHPA-2b	GP		interacts with		dose dependently			VWF	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1302_s_117	12775575	26 Whereas no binding of VWF to either rHPA-2a or rHPA-2b could be observed in the absence of ristocetin (not shown), both dose dependently interacted with VWF in the presence of 1500 mug/mL ristocetin ( Figure 3A) with a Kd,app of, respectively, 0.69 plus-or-minus 0.06 and 0.67 plus-or-minus 0.03 nmol/L (mean plus-or-minus SE) ( P=0.80), showing no statistical difference in VWF interaction at this ristocetin concentration.	bind
28093	9	7461	5	13	NULL	NULL	NULL	statement 8	Process		in the presence of					ristocetin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1302_s_117	12775575	26 Whereas no binding of VWF to either rHPA-2a or rHPA-2b could be observed in the absence of ristocetin (not shown), both dose dependently interacted with VWF in the presence of 1500 mug/mL ristocetin ( Figure 3A) with a Kd,app of, respectively, 0.69 plus-or-minus 0.06 and 0.67 plus-or-minus 0.03 nmol/L (mean plus-or-minus SE) ( P=0.80), showing no statistical difference in VWF interaction at this ristocetin concentration.	bind
30072	1	7461	7	NULL	NULL	0	NULL	VWF	NULL		does not bind	NULL				rHPA-2a	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1302_s_117	12775575	26 Whereas no binding of VWF to either rHPA-2a or rHPA-2b could be observed in the absence of ristocetin (not shown), both dose dependently interacted with VWF in the presence of 1500 mug/mL ristocetin ( Figure 3A) with a Kd,app of, respectively, 0.69 plus-or-minus 0.06 and 0.67 plus-or-minus 0.03 nmol/L (mean plus-or-minus SE) ( P=0.80), showing no statistical difference in VWF interaction at this ristocetin concentration.	bind
30073	2	7461	7	NULL	NULL	0	NULL	VWF	NULL		does not bind	NULL				rHPA-2b	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1302_s_117	12775575	26 Whereas no binding of VWF to either rHPA-2a or rHPA-2b could be observed in the absence of ristocetin (not shown), both dose dependently interacted with VWF in the presence of 1500 mug/mL ristocetin ( Figure 3A) with a Kd,app of, respectively, 0.69 plus-or-minus 0.06 and 0.67 plus-or-minus 0.03 nmol/L (mean plus-or-minus SE) ( P=0.80), showing no statistical difference in VWF interaction at this ristocetin concentration.	bind
30074	3	7461	7	NULL	NULL	0	NULL	statement 1	NULL		in absence of	NULL				ristocetin	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1302_s_117	12775575	26 Whereas no binding of VWF to either rHPA-2a or rHPA-2b could be observed in the absence of ristocetin (not shown), both dose dependently interacted with VWF in the presence of 1500 mug/mL ristocetin ( Figure 3A) with a Kd,app of, respectively, 0.69 plus-or-minus 0.06 and 0.67 plus-or-minus 0.03 nmol/L (mean plus-or-minus SE) ( P=0.80), showing no statistical difference in VWF interaction at this ristocetin concentration.	bind
30075	4	7461	7	NULL	NULL	0	NULL	statement 2	NULL		in absence of	NULL				ristocetin	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1302_s_117	12775575	26 Whereas no binding of VWF to either rHPA-2a or rHPA-2b could be observed in the absence of ristocetin (not shown), both dose dependently interacted with VWF in the presence of 1500 mug/mL ristocetin ( Figure 3A) with a Kd,app of, respectively, 0.69 plus-or-minus 0.06 and 0.67 plus-or-minus 0.03 nmol/L (mean plus-or-minus SE) ( P=0.80), showing no statistical difference in VWF interaction at this ristocetin concentration.	bind
30076	5	7461	7	NULL	NULL	0	NULL	VWF	NULL		interacts with	NULL	dose-dependently			rHPA-2a	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1302_s_117	12775575	26 Whereas no binding of VWF to either rHPA-2a or rHPA-2b could be observed in the absence of ristocetin (not shown), both dose dependently interacted with VWF in the presence of 1500 mug/mL ristocetin ( Figure 3A) with a Kd,app of, respectively, 0.69 plus-or-minus 0.06 and 0.67 plus-or-minus 0.03 nmol/L (mean plus-or-minus SE) ( P=0.80), showing no statistical difference in VWF interaction at this ristocetin concentration.	bind
30077	6	7461	7	NULL	NULL	0	NULL	VWF	NULL		interacts with	NULL	dose-dependently			rHPA-2b 	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1302_s_117	12775575	26 Whereas no binding of VWF to either rHPA-2a or rHPA-2b could be observed in the absence of ristocetin (not shown), both dose dependently interacted with VWF in the presence of 1500 mug/mL ristocetin ( Figure 3A) with a Kd,app of, respectively, 0.69 plus-or-minus 0.06 and 0.67 plus-or-minus 0.03 nmol/L (mean plus-or-minus SE) ( P=0.80), showing no statistical difference in VWF interaction at this ristocetin concentration.	bind
30078	7	7461	7	NULL	NULL	0	NULL	statement 5	NULL		in presence of	NULL				ristocetin	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1302_s_117	12775575	26 Whereas no binding of VWF to either rHPA-2a or rHPA-2b could be observed in the absence of ristocetin (not shown), both dose dependently interacted with VWF in the presence of 1500 mug/mL ristocetin ( Figure 3A) with a Kd,app of, respectively, 0.69 plus-or-minus 0.06 and 0.67 plus-or-minus 0.03 nmol/L (mean plus-or-minus SE) ( P=0.80), showing no statistical difference in VWF interaction at this ristocetin concentration.	bind
30079	8	7461	7	NULL	NULL	0	NULL	statement 6	NULL		in presence of	NULL				ristocetin	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1302_s_117	12775575	26 Whereas no binding of VWF to either rHPA-2a or rHPA-2b could be observed in the absence of ristocetin (not shown), both dose dependently interacted with VWF in the presence of 1500 mug/mL ristocetin ( Figure 3A) with a Kd,app of, respectively, 0.69 plus-or-minus 0.06 and 0.67 plus-or-minus 0.03 nmol/L (mean plus-or-minus SE) ( P=0.80), showing no statistical difference in VWF interaction at this ristocetin concentration.	bind
54520	9	7461	7	10	NULL	0	NULL	statement 1			is an alternative to					statement 2					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1302_s_117	12775575	26 Whereas no binding of VWF to either rHPA-2a or rHPA-2b could be observed in the absence of ristocetin (not shown), both dose dependently interacted with VWF in the presence of 1500 mug/mL ristocetin ( Figure 3A) with a Kd,app of, respectively, 0.69 plus-or-minus 0.06 and 0.67 plus-or-minus 0.03 nmol/L (mean plus-or-minus SE) ( P=0.80), showing no statistical difference in VWF interaction at this ristocetin concentration.	bind
28084	1	7462	5	13	NULL	NULL	NULL	p62	GP		bind					ubiquitin	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1701_s_189	10362795	26, 27  This was unexpected in view of the ubiquitin-binding capacity of normal p62.	bind
30080	1	7462	7	NULL	NULL	0	NULL	ubiquitin	NULL		bind	NULL				p62	NULL	normal			NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_6_1701_s_189	10362795	26, 27  This was unexpected in view of the ubiquitin-binding capacity of normal p62.	bind
28083	1	7463	5	13	NULL	NULL	NULL	virus	Organism		bind		effectively			PC coating	Chemical	positively charged			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_754_s_191	15681295	26,27  We confirmed effective in vitro virus binding to the positively charged PC coating.	bind
30081	1	7463	7	NULL	NULL	0	NULL	 virus	NULL		binds	NULL	effectively			PC coating	NULL	positively charged			NULL	in vitro	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_754_s_191	15681295	26,27  We confirmed effective in vitro virus binding to the positively charged PC coating.	bind
28094	1	7464	5	13	NULL	NULL	NULL	CREB	GP		bind					NOR-1	GP	close to transcription initiation point of		CRE sites	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_697_s_170	14962944	26,37  By EMSA, we show that CREB binds to the CRE sites close to the transcription initiation point of NOR-1.	bind
30082	1	7464	7	10	NULL	0	NULL	CREB	NULL		bind	NULL				NOR-1	NULL	close to the transcription initiation point		CRE site	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_697_s_170	14962944	26,37  By EMSA, we show that CREB binds to the CRE sites close to the transcription initiation point of NOR-1.	bind
28095	1	7466	5	13	NULL	NULL	NULL	26iC	GP		is a type of					murine monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_11_5357_s_187	9784544	26iC is a murine monoclonal antibody which also binds CD14 but does not block CD14-mediated activation by LPS.	bind
28096	2	7466	5	13	NULL	NULL	NULL	26iC	GP		bind					CD14	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_11_5357_s_187	9784544	26iC is a murine monoclonal antibody which also binds CD14 but does not block CD14-mediated activation by LPS.	bind
28097	3	7466	5	13	NULL	NULL	NULL	LPS	Chemical		mediate					CD14	GP	activation			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_11_5357_s_187	9784544	26iC is a murine monoclonal antibody which also binds CD14 but does not block CD14-mediated activation by LPS.	bind
28098	4	7466	5	13	NULL	NULL	NULL	26iC	GP		does not block					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_11_5357_s_187	9784544	26iC is a murine monoclonal antibody which also binds CD14 but does not block CD14-mediated activation by LPS.	bind
30085	1	7466	7	10	NULL	0	NULL	26iC	NULL	murine	binds	NULL				CD14	NULL				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_11_5357_s_187	9784544	26iC is a murine monoclonal antibody which also binds CD14 but does not block CD14-mediated activation by LPS.	bind
30086	2	7466	7	NULL	NULL	0	NULL	LPS 	NULL		mediates	NULL				CD14	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_11_5357_s_187	9784544	26iC is a murine monoclonal antibody which also binds CD14 but does not block CD14-mediated activation by LPS.	bind
30087	3	7466	7	10	NULL	0	NULL	26iC		murine	does not block					statement 2					NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_11_5357_s_187	9784544	26iC is a murine monoclonal antibody which also binds CD14 but does not block CD14-mediated activation by LPS.	bind
46615	4	7466	7	10	NULL	0	NULL	26iC	NULL		is a type of	NULL				monoclonal antibody	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_11_5357_s_187	9784544	26iC is a murine monoclonal antibody which also binds CD14 but does not block CD14-mediated activation by LPS.	bind
28102	1	7468	5	13	NULL	NULL	NULL	Ibbeta 	GP	mutation of	results in				GATA binding site of promoter	Bernard-Soulier syndrome	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_1_284_s_191	11125114	27       Ludlow,L.B., Schick,B.P., Budarf,M.L., Driscoll,D.A., Zackai,E.H., Cohen,A. and Konkle,B.A. (1996) Identification of a mutation in a GATA binding site of the platelet glycoprotein Ibbeta promoter resulting in the Bernard-Soulier syndrome.	bind
28103	2	7468	5	13	NULL	NULL	NULL	Ibbeta 	GP		is a type of					platelet glycoprotein	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_1_284_s_191	11125114	27       Ludlow,L.B., Schick,B.P., Budarf,M.L., Driscoll,D.A., Zackai,E.H., Cohen,A. and Konkle,B.A. (1996) Identification of a mutation in a GATA binding site of the platelet glycoprotein Ibbeta promoter resulting in the Bernard-Soulier syndrome.	bind
30088	1	7468	7	10	NULL	0	NULL	Ibbeta 	NULL	mutation of 	results in	NULL			GATA binding site of promoter	Bernard-Soulier syndrome	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_1_284_s_191	11125114	27       Ludlow,L.B., Schick,B.P., Budarf,M.L., Driscoll,D.A., Zackai,E.H., Cohen,A. and Konkle,B.A. (1996) Identification of a mutation in a GATA binding site of the platelet glycoprotein Ibbeta promoter resulting in the Bernard-Soulier syndrome.	bind
46616	2	7468	7	10	NULL	0	NULL	Ibbeta	NULL		is a type of	NULL				platelet glycoprotein	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_1_284_s_191	11125114	27       Ludlow,L.B., Schick,B.P., Budarf,M.L., Driscoll,D.A., Zackai,E.H., Cohen,A. and Konkle,B.A. (1996) Identification of a mutation in a GATA binding site of the platelet glycoprotein Ibbeta promoter resulting in the Bernard-Soulier syndrome.	bind
28104	1	7470	5	13	NULL	NULL	NULL	c-Myc	GP		bind		differentially			DNA	NucleicAcid	nucleosomal			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_17_3520_s_350	11522821	27       Wechsler,D.S., Papoulas,O., Dang,C.V. and Kingston,R.E. (1994) Differential binding of c-Myc and Max to nucleosomal DNA.	bind
28105	2	7470	5	13	NULL	NULL	NULL	Max	GP		bind		differentially			DNA	NucleicAcid	nucleosomal			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_17_3520_s_350	11522821	27       Wechsler,D.S., Papoulas,O., Dang,C.V. and Kingston,R.E. (1994) Differential binding of c-Myc and Max to nucleosomal DNA.	bind
30089	1	7470	7	10	NULL	0	NULL	c-Myc	NULL		binds to	NULL	differentially			DNA	NULL	nucleosomal			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_17_3520_s_350	11522821	27       Wechsler,D.S., Papoulas,O., Dang,C.V. and Kingston,R.E. (1994) Differential binding of c-Myc and Max to nucleosomal DNA.	bind
30090	2	7470	7	10	NULL	0	NULL	Max	NULL		binds to	NULL	differentially			DNA	NULL	nucleosomal			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_17_3520_s_350	11522821	27       Wechsler,D.S., Papoulas,O., Dang,C.V. and Kingston,R.E. (1994) Differential binding of c-Myc and Max to nucleosomal DNA.	bind
28099	1	7471	5	13	NULL	NULL	NULL	3H-PGI2	Chemical		bind					PGI2 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2066_s_158	9351373	27  Also the binding of 3H-PGI2 to the PGI2 receptor could be displaced by unlabeled PGE1.	bind
28100	2	7471	5	13	NULL	NULL	NULL	PGE1	Chemical	unlabeled	bind					PGI2 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2066_s_158	9351373	27  Also the binding of 3H-PGI2 to the PGI2 receptor could be displaced by unlabeled PGE1.	bind
28101	3	7471	5	13	NULL	NULL	NULL	statement 2	Process		displaces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2066_s_158	9351373	27  Also the binding of 3H-PGI2 to the PGI2 receptor could be displaced by unlabeled PGE1.	bind
30092	1	7471	7	NULL	NULL	0	NULL	3H-PGI2	NULL		binds to	NULL				PGI2 receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2066_s_158	9351373	27  Also the binding of 3H-PGI2 to the PGI2 receptor could be displaced by unlabeled PGE1.	bind
30093	2	7471	7	NULL	NULL	0	NULL	PGE1	NULL	unlabeled	binds to	NULL				PGI2 receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2066_s_158	9351373	27  Also the binding of 3H-PGI2 to the PGI2 receptor could be displaced by unlabeled PGE1.	bind
30094	3	7471	7	NULL	NULL	0	NULL	statement 2	NULL		displace	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2066_s_158	9351373	27  Also the binding of 3H-PGI2 to the PGI2 receptor could be displaced by unlabeled PGE1.	bind
28108	1	7472	5	13	NULL	NULL	NULL	hsp90	GP	binding of	is associated with					eNOS	GP	stimulation of;; activity of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2045_s_170	10978247	27  Binding of hsp90 is associated with stimulation of eNOS activity, 27  and enhanced binding of hsp90 to eNOS also appears to be involved in the estrogen receptor - mediated activation of eNOS.	bind
28109	2	7472	5	13	NULL	NULL	NULL	hsp90	GP		bind					eNOS	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2045_s_170	10978247	27  Binding of hsp90 is associated with stimulation of eNOS activity, 27  and enhanced binding of hsp90 to eNOS also appears to be involved in the estrogen receptor - mediated activation of eNOS.	bind
28110	3	7472	5	13	NULL	NULL	NULL	estrogen receptor	GP		mediate					eNOS	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2045_s_170	10978247	27  Binding of hsp90 is associated with stimulation of eNOS activity, 27  and enhanced binding of hsp90 to eNOS also appears to be involved in the estrogen receptor - mediated activation of eNOS.	bind
28111	4	7472	5	13	NULL	NULL	NULL	statement 2	Process		is involved in					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2045_s_170	10978247	27  Binding of hsp90 is associated with stimulation of eNOS activity, 27  and enhanced binding of hsp90 to eNOS also appears to be involved in the estrogen receptor - mediated activation of eNOS.	bind
30095	1	7472	7	10	NULL	0	NULL	hsp90		binding of	is associated with					eNOS		stimulation of;; activity of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2045_s_170	10978247	27  Binding of hsp90 is associated with stimulation of eNOS activity, 27  and enhanced binding of hsp90 to eNOS also appears to be involved in the estrogen receptor - mediated activation of eNOS.	bind
30096	2	7472	7	NULL	NULL	0	NULL	hsp90	NULL		binding to	NULL	enhanced			eNOS	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2045_s_170	10978247	27  Binding of hsp90 is associated with stimulation of eNOS activity, 27  and enhanced binding of hsp90 to eNOS also appears to be involved in the estrogen receptor - mediated activation of eNOS.	bind
30097	3	7472	7	NULL	NULL	0	NULL	 estrogen receptor	NULL		mediates	NULL				eNOS	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2045_s_170	10978247	27  Binding of hsp90 is associated with stimulation of eNOS activity, 27  and enhanced binding of hsp90 to eNOS also appears to be involved in the estrogen receptor - mediated activation of eNOS.	bind
30098	4	7472	7	NULL	NULL	0	NULL	statement 2	NULL		is involved in	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2045_s_170	10978247	27  Binding of hsp90 is associated with stimulation of eNOS activity, 27  and enhanced binding of hsp90 to eNOS also appears to be involved in the estrogen receptor - mediated activation of eNOS.	bind
28112	1	7473	5	13	NULL	NULL	NULL	profilin	GP		bind					VASP	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2051_s_127	10978248	27  Binding of profilin to VASP could provide a means for the local accumulation of polymerization-competent G-actin, which, in the presence of nucleating activity, can lead to filament assembly and membrane ruffling.	bind
28113	2	7473	5	13	NULL	NULL	NULL	statement 1	Process		accumulates					G-actin	GP	polymerization-competent			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2051_s_127	10978248	27  Binding of profilin to VASP could provide a means for the local accumulation of polymerization-competent G-actin, which, in the presence of nucleating activity, can lead to filament assembly and membrane ruffling.	bind
28114	3	7473	5	13	NULL	NULL	NULL	G-actin	GP		leads to					filament 	CellComponent	assembly of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2051_s_127	10978248	27  Binding of profilin to VASP could provide a means for the local accumulation of polymerization-competent G-actin, which, in the presence of nucleating activity, can lead to filament assembly and membrane ruffling.	bind
28115	4	7473	5	13	NULL	NULL	NULL	statement 3	Process		in the presence of					nucleating activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2051_s_127	10978248	27  Binding of profilin to VASP could provide a means for the local accumulation of polymerization-competent G-actin, which, in the presence of nucleating activity, can lead to filament assembly and membrane ruffling.	bind
28116	5	7473	5	13	NULL	NULL	NULL	statement 2	Process		leads to					membrane ruffling	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2051_s_127	10978248	27  Binding of profilin to VASP could provide a means for the local accumulation of polymerization-competent G-actin, which, in the presence of nucleating activity, can lead to filament assembly and membrane ruffling.	bind
28117	6	7473	5	13	NULL	NULL	NULL	statement 5	Process		in the presence of					nucleating activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2051_s_127	10978248	27  Binding of profilin to VASP could provide a means for the local accumulation of polymerization-competent G-actin, which, in the presence of nucleating activity, can lead to filament assembly and membrane ruffling.	bind
30099	1	7473	7	NULL	NULL	0	NULL	 profilin	NULL		bind	NULL				VASP	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2051_s_127	10978248	27  Binding of profilin to VASP could provide a means for the local accumulation of polymerization-competent G-actin, which, in the presence of nucleating activity, can lead to filament assembly and membrane ruffling.	bind
30100	2	7473	7	NULL	NULL	0	NULL	statement 1	NULL		accumulates	NULL	locally			G-actin	NULL	polymerization-competent			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2051_s_127	10978248	27  Binding of profilin to VASP could provide a means for the local accumulation of polymerization-competent G-actin, which, in the presence of nucleating activity, can lead to filament assembly and membrane ruffling.	bind
30101	3	7473	7	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				filament 	NULL	assembly of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2051_s_127	10978248	27  Binding of profilin to VASP could provide a means for the local accumulation of polymerization-competent G-actin, which, in the presence of nucleating activity, can lead to filament assembly and membrane ruffling.	bind
30102	4	7473	7	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				membrane ruffling	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2051_s_127	10978248	27  Binding of profilin to VASP could provide a means for the local accumulation of polymerization-competent G-actin, which, in the presence of nucleating activity, can lead to filament assembly and membrane ruffling.	bind
30103	5	7473	7	NULL	NULL	0	NULL	statement 3	NULL		in presence of	NULL				nucleating activity	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2051_s_127	10978248	27  Binding of profilin to VASP could provide a means for the local accumulation of polymerization-competent G-actin, which, in the presence of nucleating activity, can lead to filament assembly and membrane ruffling.	bind
30104	6	7473	7	NULL	NULL	0	NULL	statement 4	NULL		in presence of	NULL				nucleating activity	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2051_s_127	10978248	27  Binding of profilin to VASP could provide a means for the local accumulation of polymerization-competent G-actin, which, in the presence of nucleating activity, can lead to filament assembly and membrane ruffling.	bind
28118	1	7474	5	13	NULL	NULL	NULL	NETA	Chemical		interacts with					progesterone receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_902_s_136	9633929	27  In addition, the progestogenic effect of NETA is mediated via interaction of NETA with the progesterone receptor, 27  whereas other studies in the rabbit uterus have shown that MPA does not bind to the estrogen receptor.	bind
28119	2	7474	5	13	NULL	NULL	NULL	NETA	Chemical	progestogenic effect of	is mediated via					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_902_s_136	9633929	27  In addition, the progestogenic effect of NETA is mediated via interaction of NETA with the progesterone receptor, 27  whereas other studies in the rabbit uterus have shown that MPA does not bind to the estrogen receptor.	bind
28120	3	7474	5	13	NULL	NULL	NULL	MPA	Chemical		does not bind					estrogen receptor	GP				NULL	in rabbit uterus	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_902_s_136	9633929	27  In addition, the progestogenic effect of NETA is mediated via interaction of NETA with the progesterone receptor, 27  whereas other studies in the rabbit uterus have shown that MPA does not bind to the estrogen receptor.	bind
30105	1	7474	7	NULL	NULL	0	NULL	NETA	NULL		interacts with	NULL				progesterone receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_902_s_136	9633929	27  In addition, the progestogenic effect of NETA is mediated via interaction of NETA with the progesterone receptor, 27  whereas other studies in the rabbit uterus have shown that MPA does not bind to the estrogen receptor.	bind
30106	2	7474	7	NULL	NULL	0	NULL	statement 1	NULL		mediates	NULL				NETA	NULL	progestogenic effect of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_902_s_136	9633929	27  In addition, the progestogenic effect of NETA is mediated via interaction of NETA with the progesterone receptor, 27  whereas other studies in the rabbit uterus have shown that MPA does not bind to the estrogen receptor.	bind
30107	3	7474	7	NULL	NULL	0	NULL	MPA	NULL		does not bind	NULL				estrogen receptor 	NULL				NULL	rabbit uterus	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_902_s_136	9633929	27  In addition, the progestogenic effect of NETA is mediated via interaction of NETA with the progesterone receptor, 27  whereas other studies in the rabbit uterus have shown that MPA does not bind to the estrogen receptor.	bind
28121	1	7475	5	13	NULL	NULL	NULL	E2F-4	GP		bind					pRb2/p130	GP				NULL	G0/G1 phases in primary mouse fibroblasts	NULL	NULL	NULL	NULL	gw60_circulationres_85_11_1032_s_171	10571534	27  The main form of E2F detected in the G0/G1 phases in primary mouse fibroblasts is E2F-4 bound to pRb2/p130, which is then replaced by p107/E2F-4 complexes in late G1.	bind
28122	2	7475	5	13	NULL	NULL	NULL	E2F-4	GP		bind					p107/E2F-4 complexes	GP				NULL	late G1	NULL	NULL	NULL	NULL	gw60_circulationres_85_11_1032_s_171	10571534	27  The main form of E2F detected in the G0/G1 phases in primary mouse fibroblasts is E2F-4 bound to pRb2/p130, which is then replaced by p107/E2F-4 complexes in late G1.	bind
28123	3	7475	5	13	NULL	NULL	NULL	statement 2	Process		replaces					statement 1	Process				NULL	late G1	NULL	NULL	NULL	NULL	gw60_circulationres_85_11_1032_s_171	10571534	27  The main form of E2F detected in the G0/G1 phases in primary mouse fibroblasts is E2F-4 bound to pRb2/p130, which is then replaced by p107/E2F-4 complexes in late G1.	bind
30108	1	7475	7	NULL	NULL	0	NULL	E2F-4	NULL		bind	NULL				 pRb2/p130	NULL				NULL	G0/G1 phases in primary mouse fibroblasts	0	NULL	NULL	NULL	gw60_circulationres_85_11_1032_s_171	10571534	27  The main form of E2F detected in the G0/G1 phases in primary mouse fibroblasts is E2F-4 bound to pRb2/p130, which is then replaced by p107/E2F-4 complexes in late G1.	bind
30109	2	7475	7	NULL	NULL	0	NULL	E2F-4	NULL		bind	NULL				p107/E2F-4 complexes	NULL				NULL	late G1	NULL	NULL	NULL	NULL	gw60_circulationres_85_11_1032_s_171	10571534	27  The main form of E2F detected in the G0/G1 phases in primary mouse fibroblasts is E2F-4 bound to pRb2/p130, which is then replaced by p107/E2F-4 complexes in late G1.	bind
30110	3	7475	7	NULL	NULL	0	NULL	statement 2	NULL		replace	NULL				statement 1	NULL				NULL	late G1	0	NULL	NULL	NULL	gw60_circulationres_85_11_1032_s_171	10571534	27  The main form of E2F detected in the G0/G1 phases in primary mouse fibroblasts is E2F-4 bound to pRb2/p130, which is then replaced by p107/E2F-4 complexes in late G1.	bind
28126	1	7476	5	13	NULL	NULL	NULL			motif	is present within			WS YGVTI W		erbB1/EGFR	GP		kinase domain		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_35	10381889	27  The motif  WS YGVTI W within the kinase domain of erbB1/EGFR has been shown to be responsible for binding of this receptor tyrosine kinase to caveolins.	bind
28127	2	7476	5	13	NULL	NULL	NULL	erbB1/EGFR	GP		bind					caveolins	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_35	10381889	27  The motif  WS YGVTI W within the kinase domain of erbB1/EGFR has been shown to be responsible for binding of this receptor tyrosine kinase to caveolins.	bind
28128	3	7476	5	13	NULL	NULL	NULL	statement 1	Process		is responsible for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_35	10381889	27  The motif  WS YGVTI W within the kinase domain of erbB1/EGFR has been shown to be responsible for binding of this receptor tyrosine kinase to caveolins.	bind
28129	4	7476	5	13	NULL	NULL	NULL	erbB1/EGFR	GP		is a type of					receptor tyrosine kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_35	10381889	27  The motif  WS YGVTI W within the kinase domain of erbB1/EGFR has been shown to be responsible for binding of this receptor tyrosine kinase to caveolins.	bind
30111	1	7476	7	NULL	NULL	0	NULL		NULL		is present within	NULL		 WS YGVTI W 		erbB1/EGFR	NULL		kinase domain		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_35	10381889	27  The motif  WS YGVTI W within the kinase domain of erbB1/EGFR has been shown to be responsible for binding of this receptor tyrosine kinase to caveolins.	bind
30112	2	7476	7	NULL	NULL	0	NULL	erbB1/EGFR	NULL		bind	NULL				caveolins	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_35	10381889	27  The motif  WS YGVTI W within the kinase domain of erbB1/EGFR has been shown to be responsible for binding of this receptor tyrosine kinase to caveolins.	bind
46618	3	7476	7	NULL	NULL	0	NULL	statement 1	NULL		is responsible for	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_35	10381889	27  The motif  WS YGVTI W within the kinase domain of erbB1/EGFR has been shown to be responsible for binding of this receptor tyrosine kinase to caveolins.	bind
46619	4	7476	7	NULL	NULL	0	NULL	 erbB1/EGFR	NULL		is a type of	NULL				receptor tyrosine kinase	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_35	10381889	27  The motif  WS YGVTI W within the kinase domain of erbB1/EGFR has been shown to be responsible for binding of this receptor tyrosine kinase to caveolins.	bind
28130	1	7477	5	13	NULL	NULL	NULL				coordinate			paired cysteine residues		zinc sulfate	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_9_1282_s_227	11238274	27  This region contains paired cysteine residues that coordinate binding of a zinc sulfate, which in turn seems to be critical in maintaining the integrity of tetrahydrobiopterin binding.	bind
28131	2	7477	5	13	NULL	NULL	NULL	statement 1	Process		maintains		critical			tetrahydrobiopterin	Chemical	integrity of;;binding of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_9_1282_s_227	11238274	27  This region contains paired cysteine residues that coordinate binding of a zinc sulfate, which in turn seems to be critical in maintaining the integrity of tetrahydrobiopterin binding.	bind
30156	1	7477	7	10	NULL	0	NULL				coordinates			paired cysteine residues		zinc sulfate		binding of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_9_1282_s_227	11238274	27  This region contains paired cysteine residues that coordinate binding of a zinc sulfate, which in turn seems to be critical in maintaining the integrity of tetrahydrobiopterin binding.	bind
30157	2	7477	7	10	NULL	0	NULL	statement 1			maintains					tetrahydrobiopterin		integrity of;;binding of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_9_1282_s_227	11238274	27  This region contains paired cysteine residues that coordinate binding of a zinc sulfate, which in turn seems to be critical in maintaining the integrity of tetrahydrobiopterin binding.	bind
28132	1	7478	5	13	NULL	NULL	NULL	beta2-glycoprotein I	GP		bind					cardiolipin	Chemical	oxidized			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_108_s_113	11145941	27  We also assessed another potential cross-reactivity, which is caused by beta2-glycoprotein I binding to oxidized cardiolipin 50 ; therefore, some anti-phospholipid antibodies could react with beta2-glycoprotein I rather than oxidized phospholipids.	bind
28133	2	7478	5	13	NULL	NULL	NULL	anti-phospholipid antibodies	GP		reacts with					beta2-glycoprotein I	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_108_s_113	11145941	27  We also assessed another potential cross-reactivity, which is caused by beta2-glycoprotein I binding to oxidized cardiolipin 50 ; therefore, some anti-phospholipid antibodies could react with beta2-glycoprotein I rather than oxidized phospholipids.	bind
28134	3	7478	5	13	NULL	NULL	NULL	anti-phospholipid antibodies	GP		does not react with					phospholipids	Chemical	oxidized			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_108_s_113	11145941	27  We also assessed another potential cross-reactivity, which is caused by beta2-glycoprotein I binding to oxidized cardiolipin 50 ; therefore, some anti-phospholipid antibodies could react with beta2-glycoprotein I rather than oxidized phospholipids.	bind
30158	1	7478	7	NULL	NULL	0	NULL	beta2-glycoprotein I	NULL		bind	NULL				cardiolipin 50	NULL	oxidized			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_108_s_113	11145941	27  We also assessed another potential cross-reactivity, which is caused by beta2-glycoprotein I binding to oxidized cardiolipin 50 ; therefore, some anti-phospholipid antibodies could react with beta2-glycoprotein I rather than oxidized phospholipids.	bind
30159	2	7478	7	NULL	NULL	0	NULL	anti-phospholipid antibodies	NULL		react with	NULL				beta2-glycoprotein I	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_108_s_113	11145941	27  We also assessed another potential cross-reactivity, which is caused by beta2-glycoprotein I binding to oxidized cardiolipin 50 ; therefore, some anti-phospholipid antibodies could react with beta2-glycoprotein I rather than oxidized phospholipids.	bind
30160	3	7478	7	10	NULL	0	NULL	anti-phospholipid antibodies			does not react with					phospholipids		oxidized			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_1_108_s_113	11145941	27  We also assessed another potential cross-reactivity, which is caused by beta2-glycoprotein I binding to oxidized cardiolipin 50 ; therefore, some anti-phospholipid antibodies could react with beta2-glycoprotein I rather than oxidized phospholipids.	bind
28135	1	7479	5	13	NULL	NULL	NULL	Lp(a)	GP	levels of plasma	decline during					sepsis	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1137_s_120	10764684	27 31  In the present study, plasma concentrations of free apo(a), which comprises apo(a) fragments and full-length apo(a) not bound to LDL particles, and urinary apo(a) levels remained unchanged during the study period, indicating that the decline in plasma Lp(a) levels during sepsis and burns was probably not due to accelerated fragmentation of apo(a) in plasma.	bind
28136	2	7479	5	13	NULL	NULL	NULL	Lp(a)	GP	levels of plasma	decline during					burns	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1137_s_120	10764684	27 31  In the present study, plasma concentrations of free apo(a), which comprises apo(a) fragments and full-length apo(a) not bound to LDL particles, and urinary apo(a) levels remained unchanged during the study period, indicating that the decline in plasma Lp(a) levels during sepsis and burns was probably not due to accelerated fragmentation of apo(a) in plasma.	bind
28137	3	7479	5	13	NULL	NULL	NULL	apo(a)	GP	accelerated fragmentation of	does not cause		probably			statement 1	Process				NULL	in plasma	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1137_s_120	10764684	27 31  In the present study, plasma concentrations of free apo(a), which comprises apo(a) fragments and full-length apo(a) not bound to LDL particles, and urinary apo(a) levels remained unchanged during the study period, indicating that the decline in plasma Lp(a) levels during sepsis and burns was probably not due to accelerated fragmentation of apo(a) in plasma.	bind
28138	4	7479	5	13	NULL	NULL	NULL	apo(a)	GP	accelerated fragmentation of	does not cause		probably			statement 2	Process				NULL	in plasma	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1137_s_120	10764684	27 31  In the present study, plasma concentrations of free apo(a), which comprises apo(a) fragments and full-length apo(a) not bound to LDL particles, and urinary apo(a) levels remained unchanged during the study period, indicating that the decline in plasma Lp(a) levels during sepsis and burns was probably not due to accelerated fragmentation of apo(a) in plasma.	bind
30162	1	7479	7	NULL	NULL	0	NULL	apo(a)	NULL		does not bind	NULL				LDL particles	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1137_s_120	10764684	27 31  In the present study, plasma concentrations of free apo(a), which comprises apo(a) fragments and full-length apo(a) not bound to LDL particles, and urinary apo(a) levels remained unchanged during the study period, indicating that the decline in plasma Lp(a) levels during sepsis and burns was probably not due to accelerated fragmentation of apo(a) in plasma.	bind
30165	2	7479	7	10	NULL	0	NULL	apo(a)			undergoes					fragmentation		accelerated			NULL	plasma	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1137_s_120	10764684	27 31  In the present study, plasma concentrations of free apo(a), which comprises apo(a) fragments and full-length apo(a) not bound to LDL particles, and urinary apo(a) levels remained unchanged during the study period, indicating that the decline in plasma Lp(a) levels during sepsis and burns was probably not due to accelerated fragmentation of apo(a) in plasma.	bind
30166	3	7479	7	10	NULL	0	NULL	Lp(a)		plasma levels of	decline during					sepsis					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1137_s_120	10764684	27 31  In the present study, plasma concentrations of free apo(a), which comprises apo(a) fragments and full-length apo(a) not bound to LDL particles, and urinary apo(a) levels remained unchanged during the study period, indicating that the decline in plasma Lp(a) levels during sepsis and burns was probably not due to accelerated fragmentation of apo(a) in plasma.	bind
30167	4	7479	7	10	NULL	0	NULL	Lp(a)		plasma levels of	decline during					burns					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1137_s_120	10764684	27 31  In the present study, plasma concentrations of free apo(a), which comprises apo(a) fragments and full-length apo(a) not bound to LDL particles, and urinary apo(a) levels remained unchanged during the study period, indicating that the decline in plasma Lp(a) levels during sepsis and burns was probably not due to accelerated fragmentation of apo(a) in plasma.	bind
30168	5	7479	7	10	NULL	0	NULL	statement 3			is not due to		probably			statement 2					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1137_s_120	10764684	27 31  In the present study, plasma concentrations of free apo(a), which comprises apo(a) fragments and full-length apo(a) not bound to LDL particles, and urinary apo(a) levels remained unchanged during the study period, indicating that the decline in plasma Lp(a) levels during sepsis and burns was probably not due to accelerated fragmentation of apo(a) in plasma.	bind
30169	6	7479	7	10	NULL	0	NULL	statement 4			is not due to		probably			statement 2					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_4_1137_s_120	10764684	27 31  In the present study, plasma concentrations of free apo(a), which comprises apo(a) fragments and full-length apo(a) not bound to LDL particles, and urinary apo(a) levels remained unchanged during the study period, indicating that the decline in plasma Lp(a) levels during sepsis and burns was probably not due to accelerated fragmentation of apo(a) in plasma.	bind
28139	1	7480	5	13	NULL	NULL	NULL	HSP27	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_2_192_s_167	15976317	27 As well as binding to actin, HSP27 also binds to the intermediate filament vimentin.	bind
28140	2	7480	5	13	NULL	NULL	NULL	HSP27	GP		bind					vimentin	GP	intermediate filament			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_2_192_s_167	15976317	27 As well as binding to actin, HSP27 also binds to the intermediate filament vimentin.	bind
30170	1	7480	7	NULL	NULL	0	NULL	HSP27	NULL		binds to	NULL				actin	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_2_192_s_167	15976317	27 As well as binding to actin, HSP27 also binds to the intermediate filament vimentin.	bind
30171	2	7480	7	NULL	NULL	0	NULL	HSP27	NULL		binds to	NULL				 vimentin	NULL	intermediate filament			NULL		0	NULL	NULL	NULL	gw70_circulationres_97_2_192_s_167	15976317	27 As well as binding to actin, HSP27 also binds to the intermediate filament vimentin.	bind
28141	1	7483	5	13	NULL	NULL	NULL	SRF	GP		bind									CArG box	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1602_s_213	15242862	27 Further investigation of the molecular basis for enhancement of the binding of SRF to CArG box by Hex will provide the clue for the understanding of the context-dependent and signal-responsive regulation of phenotypic modulation of vascular SMC.	bind
46617	2	7483	5	13	NULL	NULL	NULL	Hex	GP		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1602_s_213	15242862	27 Further investigation of the molecular basis for enhancement of the binding of SRF to CArG box by Hex will provide the clue for the understanding of the context-dependent and signal-responsive regulation of phenotypic modulation of vascular SMC.	bind
30172	1	7483	7	NULL	NULL	0	NULL	 SRF	NULL		binds to	NULL					NULL			CArG box 	NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1602_s_213	15242862	27 Further investigation of the molecular basis for enhancement of the binding of SRF to CArG box by Hex will provide the clue for the understanding of the context-dependent and signal-responsive regulation of phenotypic modulation of vascular SMC.	bind
54521	2	7483	7	10	NULL	0	NULL	Hex			enhances					statement 1					NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1602_s_213	15242862	27 Further investigation of the molecular basis for enhancement of the binding of SRF to CArG box by Hex will provide the clue for the understanding of the context-dependent and signal-responsive regulation of phenotypic modulation of vascular SMC.	bind
28143	1	7484	5	13	NULL	NULL	NULL	LpL	GP		function within		potential			arterial wall	OrganismPart	mouse			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1333_s_179	12089072	27 LpL also could potentially function within the mouse arterial wall to facilitate non - proteoglycan-mediated HDL3-E binding, because LpL may bind to HDL through lipophilic interactions that are independent of apo E. 28	bind
28144	2	7484	5	13	NULL	NULL	NULL	non - proteoglycan	GP		mediates					HDL3-E	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1333_s_179	12089072	27 LpL also could potentially function within the mouse arterial wall to facilitate non - proteoglycan-mediated HDL3-E binding, because LpL may bind to HDL through lipophilic interactions that are independent of apo E. 28	bind
28145	3	7484	5	13	NULL	NULL	NULL	LpL	GP		bind		may			HDL	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1333_s_179	12089072	27 LpL also could potentially function within the mouse arterial wall to facilitate non - proteoglycan-mediated HDL3-E binding, because LpL may bind to HDL through lipophilic interactions that are independent of apo E. 28	bind
28146	4	7484	5	13	NULL	NULL	NULL	lipophilic interactions	Process		is independent of					apo E	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1333_s_179	12089072	27 LpL also could potentially function within the mouse arterial wall to facilitate non - proteoglycan-mediated HDL3-E binding, because LpL may bind to HDL through lipophilic interactions that are independent of apo E. 28	bind
28147	5	7484	5	13	NULL	NULL	NULL	statement 3	Process		occurs through					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1333_s_179	12089072	27 LpL also could potentially function within the mouse arterial wall to facilitate non - proteoglycan-mediated HDL3-E binding, because LpL may bind to HDL through lipophilic interactions that are independent of apo E. 28	bind
30177	1	7484	7	NULL	NULL	0	NULL	 LpL	NULL		bind	NULL	may			HDL	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_12_1333_s_179	12089072	27 LpL also could potentially function within the mouse arterial wall to facilitate non - proteoglycan-mediated HDL3-E binding, because LpL may bind to HDL through lipophilic interactions that are independent of apo E. 28	bind
30178	2	7484	7	NULL	NULL	0	NULL	statement 1	NULL		occurs through	NULL				lipophilic interactions	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_12_1333_s_179	12089072	27 LpL also could potentially function within the mouse arterial wall to facilitate non - proteoglycan-mediated HDL3-E binding, because LpL may bind to HDL through lipophilic interactions that are independent of apo E. 28	bind
30179	3	7484	7	NULL	NULL	0	NULL	statement 1	NULL		is independent of	NULL				apo E	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_12_1333_s_179	12089072	27 LpL also could potentially function within the mouse arterial wall to facilitate non - proteoglycan-mediated HDL3-E binding, because LpL may bind to HDL through lipophilic interactions that are independent of apo E. 28	bind
30180	4	7484	7	NULL	NULL	0	NULL	LpL	NULL		function within	NULL	potentially			arterial wall 	NULL	mouse			NULL		0	NULL	NULL	NULL	gw60_circulationres_90_12_1333_s_179	12089072	27 LpL also could potentially function within the mouse arterial wall to facilitate non - proteoglycan-mediated HDL3-E binding, because LpL may bind to HDL through lipophilic interactions that are independent of apo E. 28	bind
30181	5	7484	7	NULL	NULL	0	NULL	non - proteoglycan	NULL		mediates	NULL				HDL3-E	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_circulationres_90_12_1333_s_179	12089072	27 LpL also could potentially function within the mouse arterial wall to facilitate non - proteoglycan-mediated HDL3-E binding, because LpL may bind to HDL through lipophilic interactions that are independent of apo E. 28	bind
30182	6	7484	7	NULL	NULL	0	NULL	statement 4	NULL		facilitate	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_12_1333_s_179	12089072	27 LpL also could potentially function within the mouse arterial wall to facilitate non - proteoglycan-mediated HDL3-E binding, because LpL may bind to HDL through lipophilic interactions that are independent of apo E. 28	bind
30183	7	7484	7	NULL	NULL	0	NULL	statement 6	NULL		is because of 	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_12_1333_s_179	12089072	27 LpL also could potentially function within the mouse arterial wall to facilitate non - proteoglycan-mediated HDL3-E binding, because LpL may bind to HDL through lipophilic interactions that are independent of apo E. 28	bind
28148	1	7485	5	13	NULL	NULL	NULL	NFATc1	GP		bind			Rel homology domain		DNA	NucleicAcid			consensus sequence	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1492_s_185	15117818	27 NFATc1 - NFATc4 bind the consensus DNA sequence through a Rel homology domain, and all 4 of these factors are expressed in cardiac myocytes.	bind
46685	2	7485	5	13	NULL	NULL	NULL	NFATc2	GP		bind			Rel homology domain		DNA	NucleicAcid			consensus sequence	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1492_s_185	15117818	27 NFATc1 - NFATc4 bind the consensus DNA sequence through a Rel homology domain, and all 4 of these factors are expressed in cardiac myocytes.	bind
46686	3	7485	5	13	NULL	NULL	NULL	NFATc3	GP		bind			Rel homology domain		DNA	NucleicAcid			consensus sequence	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1492_s_185	15117818	27 NFATc1 - NFATc4 bind the consensus DNA sequence through a Rel homology domain, and all 4 of these factors are expressed in cardiac myocytes.	bind
46687	4	7485	5	13	NULL	NULL	NULL	NFATc4	GP		bind			Rel homology domain		DNA	NucleicAcid			consensus sequence	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1492_s_185	15117818	27 NFATc1 - NFATc4 bind the consensus DNA sequence through a Rel homology domain, and all 4 of these factors are expressed in cardiac myocytes.	bind
46688	5	7485	5	13	NULL	NULL	NULL	NFATc1	GP		is expressed in					cardiac myocytes	Cell				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1492_s_185	15117818	27 NFATc1 - NFATc4 bind the consensus DNA sequence through a Rel homology domain, and all 4 of these factors are expressed in cardiac myocytes.	bind
46689	6	7485	5	13	NULL	NULL	NULL	NFATc2	GP		is expressed in					cardiac myocytes	Cell				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1492_s_185	15117818	27 NFATc1 - NFATc4 bind the consensus DNA sequence through a Rel homology domain, and all 4 of these factors are expressed in cardiac myocytes.	bind
46690	7	7485	5	13	NULL	NULL	NULL	NFATc3	GP		is expressed in					cardiac myocytes	Cell				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1492_s_185	15117818	27 NFATc1 - NFATc4 bind the consensus DNA sequence through a Rel homology domain, and all 4 of these factors are expressed in cardiac myocytes.	bind
46691	8	7485	5	13	NULL	NULL	NULL	NFATc4	GP		is expressed in					cardiac myocytes	Cell				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1492_s_185	15117818	27 NFATc1 - NFATc4 bind the consensus DNA sequence through a Rel homology domain, and all 4 of these factors are expressed in cardiac myocytes.	bind
30184	1	7485	7	NULL	NULL	0	NULL	NFATc1	NULL		bind	NULL		Rel homology domain		DNA	NULL			consensus sequence	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1492_s_185	15117818	27 NFATc1 - NFATc4 bind the consensus DNA sequence through a Rel homology domain, and all 4 of these factors are expressed in cardiac myocytes.	bind
30185	2	7485	7	NULL	NULL	0	NULL	NFATc2	NULL		bind	NULL		Rel homology domain		DNA	NULL			consensus sequence	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1492_s_185	15117818	27 NFATc1 - NFATc4 bind the consensus DNA sequence through a Rel homology domain, and all 4 of these factors are expressed in cardiac myocytes.	bind
30186	3	7485	7	NULL	NULL	0	NULL	NFATc3	NULL		bind	NULL		Rel homology domain		DNA	NULL			consensus sequence	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1492_s_185	15117818	27 NFATc1 - NFATc4 bind the consensus DNA sequence through a Rel homology domain, and all 4 of these factors are expressed in cardiac myocytes.	bind
30187	4	7485	7	NULL	NULL	0	NULL	NFATc4	NULL		bind	NULL		Rel homology domain		DNA	NULL			consensus sequence	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1492_s_185	15117818	27 NFATc1 - NFATc4 bind the consensus DNA sequence through a Rel homology domain, and all 4 of these factors are expressed in cardiac myocytes.	bind
30188	5	7485	7	NULL	NULL	0	NULL	NFATc1	NULL		is expressed in	NULL				cardiac myocytes	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_11_1492_s_185	15117818	27 NFATc1 - NFATc4 bind the consensus DNA sequence through a Rel homology domain, and all 4 of these factors are expressed in cardiac myocytes.	bind
30189	6	7485	7	NULL	NULL	0	NULL	NFATc2	NULL		is expressed in	NULL				cardiac myocytes	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_11_1492_s_185	15117818	27 NFATc1 - NFATc4 bind the consensus DNA sequence through a Rel homology domain, and all 4 of these factors are expressed in cardiac myocytes.	bind
30190	7	7485	7	NULL	NULL	0	NULL	NFATc3	NULL		is expressed in	NULL				cardiac myocytes	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_11_1492_s_185	15117818	27 NFATc1 - NFATc4 bind the consensus DNA sequence through a Rel homology domain, and all 4 of these factors are expressed in cardiac myocytes.	bind
30191	8	7485	7	NULL	NULL	0	NULL	NFATc4	NULL		is expressed in	NULL				cardiac myocytes	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_11_1492_s_185	15117818	27 NFATc1 - NFATc4 bind the consensus DNA sequence through a Rel homology domain, and all 4 of these factors are expressed in cardiac myocytes.	bind
28149	1	7486	5	13	NULL	NULL	NULL	PKCzeta atypical isoform	GP		prevents					IkappaBalpha	GP	degradation of			NULL	in TNF-stimulated endothelial cells	NULL	NULL	NULL	NULL	gw60_circulationres_92_10_1130_s_194	12714566	27 Rahman et al, 27 using a dominant-negative approach, were able to demonstrate in TNF-stimulated endothelial cells that the atypical isoform PKCzeta was able to prevent IkappaBalpha degradation and NF-kappaB binding to the ICAM-1 promoter.	bind
28150	2	7486	5	13	NULL	NULL	NULL	NF-kappaB	GP		bind					ICAM-1	GP			promoter	NULL	TNF-stimulated endothelial cells	NULL	NULL	NULL	NULL	gw60_circulationres_92_10_1130_s_194	12714566	27 Rahman et al, 27 using a dominant-negative approach, were able to demonstrate in TNF-stimulated endothelial cells that the atypical isoform PKCzeta was able to prevent IkappaBalpha degradation and NF-kappaB binding to the ICAM-1 promoter.	bind
28151	3	7486	5	13	NULL	NULL	NULL	PKCzeta atypical isoform	GP		prevents					statement 2	Process				NULL	TNF-stimulated endothelial cells	NULL	NULL	NULL	NULL	gw60_circulationres_92_10_1130_s_194	12714566	27 Rahman et al, 27 using a dominant-negative approach, were able to demonstrate in TNF-stimulated endothelial cells that the atypical isoform PKCzeta was able to prevent IkappaBalpha degradation and NF-kappaB binding to the ICAM-1 promoter.	bind
30192	1	7486	7	10	NULL	0	NULL	NF-kappaB			binds to					ICAM-1				promoter	NULL	TNF-stimulated endothelial cells	NULL	NULL	NULL	NULL	gw60_circulationres_92_10_1130_s_194	12714566	27 Rahman et al, 27 using a dominant-negative approach, were able to demonstrate in TNF-stimulated endothelial cells that the atypical isoform PKCzeta was able to prevent IkappaBalpha degradation and NF-kappaB binding to the ICAM-1 promoter.	bind
30194	2	7486	7	10	NULL	0	NULL	PKCzeta atypical isoform			prevent					IkappaBalpha 		degradation of			NULL	TNF-stimulated endothelial cells	NULL	NULL	NULL	NULL	gw60_circulationres_92_10_1130_s_194	12714566	27 Rahman et al, 27 using a dominant-negative approach, were able to demonstrate in TNF-stimulated endothelial cells that the atypical isoform PKCzeta was able to prevent IkappaBalpha degradation and NF-kappaB binding to the ICAM-1 promoter.	bind
30195	3	7486	7	10	NULL	0	NULL	PKCzeta atypical isoform			prevents					statement 1					NULL	TNF-stimulated endothelial cells	NULL	NULL	NULL	NULL	gw60_circulationres_92_10_1130_s_194	12714566	27 Rahman et al, 27 using a dominant-negative approach, were able to demonstrate in TNF-stimulated endothelial cells that the atypical isoform PKCzeta was able to prevent IkappaBalpha degradation and NF-kappaB binding to the ICAM-1 promoter.	bind
28152	1	7487	5	13	NULL	NULL	NULL	WT1	GP		represses					PAX2	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_amjpathol_154_1_181_s_44	9916932	27 Repression of  PAX2 by WT1 has been demonstrated  in vitro by the binding of WT1 to  PAX2 regulatory sequences and by cotransfection assays using CAT reporter constructs under the control of  PAX2 regulatory sequences showing WT1-dependent transcriptional repression.	bind
28153	2	7487	5	13	NULL	NULL	NULL	WT1	GP		bind					PAX2	GP			regulatory sequences	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_amjpathol_154_1_181_s_44	9916932	27 Repression of  PAX2 by WT1 has been demonstrated  in vitro by the binding of WT1 to  PAX2 regulatory sequences and by cotransfection assays using CAT reporter constructs under the control of  PAX2 regulatory sequences showing WT1-dependent transcriptional repression.	bind
28154	3	7487	5	13	NULL	NULL	NULL	statement 2	Process		leads to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_1_181_s_44	9916932	27 Repression of  PAX2 by WT1 has been demonstrated  in vitro by the binding of WT1 to  PAX2 regulatory sequences and by cotransfection assays using CAT reporter constructs under the control of  PAX2 regulatory sequences showing WT1-dependent transcriptional repression.	bind
30196	1	7487	7	NULL	NULL	0	NULL	WT1	NULL		bind	NULL				PAX2	NULL			regulatory sequences	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_amjpathol_154_1_181_s_44	9916932	27 Repression of  PAX2 by WT1 has been demonstrated  in vitro by the binding of WT1 to  PAX2 regulatory sequences and by cotransfection assays using CAT reporter constructs under the control of  PAX2 regulatory sequences showing WT1-dependent transcriptional repression.	bind
30197	2	7487	7	NULL	NULL	0	NULL	statement 1	NULL		repress	NULL				PAX2	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_amjpathol_154_1_181_s_44	9916932	27 Repression of  PAX2 by WT1 has been demonstrated  in vitro by the binding of WT1 to  PAX2 regulatory sequences and by cotransfection assays using CAT reporter constructs under the control of  PAX2 regulatory sequences showing WT1-dependent transcriptional repression.	bind
30198	3	7487	7	NULL	NULL	0	NULL	transcription	NULL	repression of	depends on	NULL				WT1	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_1_181_s_44	9916932	27 Repression of  PAX2 by WT1 has been demonstrated  in vitro by the binding of WT1 to  PAX2 regulatory sequences and by cotransfection assays using CAT reporter constructs under the control of  PAX2 regulatory sequences showing WT1-dependent transcriptional repression.	bind
30199	4	7487	7	NULL	NULL	0	NULL	PAX2	NULL	control of	show	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_1_181_s_44	9916932	27 Repression of  PAX2 by WT1 has been demonstrated  in vitro by the binding of WT1 to  PAX2 regulatory sequences and by cotransfection assays using CAT reporter constructs under the control of  PAX2 regulatory sequences showing WT1-dependent transcriptional repression.	bind
28155	1	7488	5	13	NULL	NULL	NULL	DNA	NucleicAcid	adenovirus	bind					VCAM-1+ cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_2_238_s_98	11156859	27 There was  3-fold more adenovirus DNA bound to VCAM-1+ cells (2.7 plus-or-minus 0.8, n=3) than to parental NIH 3T3 cells (1 plus-or-minus 0, n=3; Figure 5  ).	bind
28156	2	7488	5	13	NULL	NULL	NULL	DNA	NucleicAcid	adenovirus	bind					NIH 3T3 cells	Cell	parental			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_2_238_s_98	11156859	27 There was  3-fold more adenovirus DNA bound to VCAM-1+ cells (2.7 plus-or-minus 0.8, n=3) than to parental NIH 3T3 cells (1 plus-or-minus 0, n=3; Figure 5  ).	bind
28157	3	7488	5	13	NULL	NULL	NULL	statement 1	Process	binding of	is more than					statement 2	Process	binding of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_2_238_s_98	11156859	27 There was  3-fold more adenovirus DNA bound to VCAM-1+ cells (2.7 plus-or-minus 0.8, n=3) than to parental NIH 3T3 cells (1 plus-or-minus 0, n=3; Figure 5  ).	bind
30200	1	7488	7	NULL	NULL	0	NULL	DNA	NULL	adenovirus 	bind	NULL				VCAM-1+ cells	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_2_238_s_98	11156859	27 There was  3-fold more adenovirus DNA bound to VCAM-1+ cells (2.7 plus-or-minus 0.8, n=3) than to parental NIH 3T3 cells (1 plus-or-minus 0, n=3; Figure 5  ).	bind
30201	2	7488	7	NULL	NULL	0	NULL	DNA	NULL	adenovirus 	bind	NULL				NIH 3T3 cells	NULL	parental			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_2_238_s_98	11156859	27 There was  3-fold more adenovirus DNA bound to VCAM-1+ cells (2.7 plus-or-minus 0.8, n=3) than to parental NIH 3T3 cells (1 plus-or-minus 0, n=3; Figure 5  ).	bind
30202	3	7488	7	10	NULL	0	NULL	statement 1	NULL	binding of	is greater than	NULL				statement 2	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_2_238_s_98	11156859	27 There was  3-fold more adenovirus DNA bound to VCAM-1+ cells (2.7 plus-or-minus 0.8, n=3) than to parental NIH 3T3 cells (1 plus-or-minus 0, n=3; Figure 5  ).	bind
28158	1	7489	5	13	NULL	NULL	NULL	apoA-I	GP		bind		directly			ABCA1	GP				NULL	at the cell surface	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_53	12738681	27 These findings have been confirmed independently 30,31  and strongly suggested that apoA-I directly binds ABCA1 at the cell surface without requiring the ability of ABCA1 to mediate lipid efflux.	bind
28159	2	7489	5	13	NULL	NULL	NULL	ABCA1	GP		mediate					lipid efflux	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_53	12738681	27 These findings have been confirmed independently 30,31  and strongly suggested that apoA-I directly binds ABCA1 at the cell surface without requiring the ability of ABCA1 to mediate lipid efflux.	bind
28160	3	7489	5	13	NULL	NULL	NULL	statement 1	Process		does not require					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_53	12738681	27 These findings have been confirmed independently 30,31  and strongly suggested that apoA-I directly binds ABCA1 at the cell surface without requiring the ability of ABCA1 to mediate lipid efflux.	bind
30203	1	7489	7	NULL	NULL	0	NULL	apoA-I 	NULL		binds	NULL	directly			ABCA1	NULL				NULL	cell surface	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_53	12738681	27 These findings have been confirmed independently 30,31  and strongly suggested that apoA-I directly binds ABCA1 at the cell surface without requiring the ability of ABCA1 to mediate lipid efflux.	bind
30204	2	7489	7	NULL	NULL	0	NULL	ABCA1	NULL		mediate	NULL				lipid efflux	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_53	12738681	27 These findings have been confirmed independently 30,31  and strongly suggested that apoA-I directly binds ABCA1 at the cell surface without requiring the ability of ABCA1 to mediate lipid efflux.	bind
30205	3	7489	7	NULL	NULL	0	NULL	statement 1	NULL		does not require	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_53	12738681	27 These findings have been confirmed independently 30,31  and strongly suggested that apoA-I directly binds ABCA1 at the cell surface without requiring the ability of ABCA1 to mediate lipid efflux.	bind
28161	1	7490	5	13	NULL	NULL	NULL	MecI	GP	purified	bind					DNA bla	NucleicAcid			135bp operator containing inter blaZ - blaR1 sequence	NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_47_4_377_s_108	11266408	27 To investigate by the same technique whether or not there are differences between the sites on the  bla operators that are bound by MecI and BlaI, the purified proteins were bound to the 135 bp DNA  bla operator probe, which contains the inter  blaZ - blaR1 sequence.	bind
28162	2	7490	5	13	NULL	NULL	NULL	BlaI	GP	purified	bind					DNA bla	NucleicAcid			135bp operator containing inter blaZ - blaR1 sequence	NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_47_4_377_s_108	11266408	27 To investigate by the same technique whether or not there are differences between the sites on the  bla operators that are bound by MecI and BlaI, the purified proteins were bound to the 135 bp DNA  bla operator probe, which contains the inter  blaZ - blaR1 sequence.	bind
30206	1	7490	7	10	NULL	0	NULL	MecI	NULL	purified	bind	NULL				DNA bla	NULL			135bp operator containing inter blaZ - blaR1 sequence	NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_47_4_377_s_108	11266408	27 To investigate by the same technique whether or not there are differences between the sites on the  bla operators that are bound by MecI and BlaI, the purified proteins were bound to the 135 bp DNA  bla operator probe, which contains the inter  blaZ - blaR1 sequence.	bind
30207	2	7490	7	10	NULL	0	NULL	BlaI	NULL	purified	bind	NULL				DNA bla	NULL			135bp operator containing inter blaZ - blaR1 sequence	NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_47_4_377_s_108	11266408	27 To investigate by the same technique whether or not there are differences between the sites on the  bla operators that are bound by MecI and BlaI, the purified proteins were bound to the 135 bp DNA  bla operator probe, which contains the inter  blaZ - blaR1 sequence.	bind
28163	1	7491	5	13	NULL	NULL	NULL	TNF-alpha	GP		bind					collagen	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_12	12000736	27, 28 It is well recognized that TNF-alpha binds to ECM proteins, including collagen, fibronectin, and laminin, 31- 33  which constitute the main matrix components of epiretinal membranes.	bind
28164	2	7491	5	13	NULL	NULL	NULL	TNF-alpha	GP		bind					fibronectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_12	12000736	27, 28 It is well recognized that TNF-alpha binds to ECM proteins, including collagen, fibronectin, and laminin, 31- 33  which constitute the main matrix components of epiretinal membranes.	bind
28165	3	7491	5	13	NULL	NULL	NULL	TNF-alpha	GP		bind					laminin	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_12	12000736	27, 28 It is well recognized that TNF-alpha binds to ECM proteins, including collagen, fibronectin, and laminin, 31- 33  which constitute the main matrix components of epiretinal membranes.	bind
28166	4	7491	5	13	NULL	NULL	NULL	collagen	GP		is a type of					ECM proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_12	12000736	27, 28 It is well recognized that TNF-alpha binds to ECM proteins, including collagen, fibronectin, and laminin, 31- 33  which constitute the main matrix components of epiretinal membranes.	bind
28167	5	7491	5	13	NULL	NULL	NULL	fibronectin	GP		is a type of					ECM proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_12	12000736	27, 28 It is well recognized that TNF-alpha binds to ECM proteins, including collagen, fibronectin, and laminin, 31- 33  which constitute the main matrix components of epiretinal membranes.	bind
28168	6	7491	5	13	NULL	NULL	NULL	laminin	GP		is a type of					ECM proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_12	12000736	27, 28 It is well recognized that TNF-alpha binds to ECM proteins, including collagen, fibronectin, and laminin, 31- 33  which constitute the main matrix components of epiretinal membranes.	bind
28169	7	7491	5	13	NULL	NULL	NULL	collagen	GP		constitutes					epiretinal membranes	OrganismPart	main matrix components of 			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_12	12000736	27, 28 It is well recognized that TNF-alpha binds to ECM proteins, including collagen, fibronectin, and laminin, 31- 33  which constitute the main matrix components of epiretinal membranes.	bind
28170	8	7491	5	13	NULL	NULL	NULL	fibronectin	GP		constitutes					epiretinal membranes	OrganismPart	main matrix components of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_12	12000736	27, 28 It is well recognized that TNF-alpha binds to ECM proteins, including collagen, fibronectin, and laminin, 31- 33  which constitute the main matrix components of epiretinal membranes.	bind
28171	9	7491	5	13	NULL	NULL	NULL	laminin	GP		constitutes					epiretinal membranes	OrganismPart	main matrix components of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_12	12000736	27, 28 It is well recognized that TNF-alpha binds to ECM proteins, including collagen, fibronectin, and laminin, 31- 33  which constitute the main matrix components of epiretinal membranes.	bind
30208	1	7491	7	NULL	NULL	0	NULL	TNF-alpha	NULL		bind	NULL				collagen	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_12	12000736	27, 28 It is well recognized that TNF-alpha binds to ECM proteins, including collagen, fibronectin, and laminin, 31- 33  which constitute the main matrix components of epiretinal membranes.	bind
30209	2	7491	7	NULL	NULL	0	NULL	TNF-alpha	NULL		bind	NULL				fibronectin	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_12	12000736	27, 28 It is well recognized that TNF-alpha binds to ECM proteins, including collagen, fibronectin, and laminin, 31- 33  which constitute the main matrix components of epiretinal membranes.	bind
30210	3	7491	7	NULL	NULL	0	NULL	TNF-alpha	NULL		bind	NULL				laminin	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_12	12000736	27, 28 It is well recognized that TNF-alpha binds to ECM proteins, including collagen, fibronectin, and laminin, 31- 33  which constitute the main matrix components of epiretinal membranes.	bind
30211	4	7491	7	NULL	NULL	0	NULL	collagen	NULL		is a type of	NULL				ECM protein	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_12	12000736	27, 28 It is well recognized that TNF-alpha binds to ECM proteins, including collagen, fibronectin, and laminin, 31- 33  which constitute the main matrix components of epiretinal membranes.	bind
30212	5	7491	7	NULL	NULL	0	NULL	fibronectin	NULL		is a type of	NULL				ECM protein	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_12	12000736	27, 28 It is well recognized that TNF-alpha binds to ECM proteins, including collagen, fibronectin, and laminin, 31- 33  which constitute the main matrix components of epiretinal membranes.	bind
30213	6	7491	7	NULL	NULL	0	NULL	laminin	NULL		is a type of	NULL				ECM protein	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_12	12000736	27, 28 It is well recognized that TNF-alpha binds to ECM proteins, including collagen, fibronectin, and laminin, 31- 33  which constitute the main matrix components of epiretinal membranes.	bind
30214	7	7491	7	NULL	NULL	0	NULL	collagen	NULL		constitute 	NULL				epiretinal membrane	NULL	main matrix component of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_12	12000736	27, 28 It is well recognized that TNF-alpha binds to ECM proteins, including collagen, fibronectin, and laminin, 31- 33  which constitute the main matrix components of epiretinal membranes.	bind
30215	8	7491	7	NULL	NULL	0	NULL	fibronectin	NULL		constitute 	NULL				epiretinal membrane	NULL	main matrix component of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_12	12000736	27, 28 It is well recognized that TNF-alpha binds to ECM proteins, including collagen, fibronectin, and laminin, 31- 33  which constitute the main matrix components of epiretinal membranes.	bind
30216	9	7491	7	NULL	NULL	0	NULL	laminin	NULL		constitute 	NULL				epiretinal membrane	NULL	main matrix component of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_12	12000736	27, 28 It is well recognized that TNF-alpha binds to ECM proteins, including collagen, fibronectin, and laminin, 31- 33  which constitute the main matrix components of epiretinal membranes.	bind
30145	1	7492	5	13	NULL	NULL	NULL	plasma gammaA/gamma'' fibrinogen	GP	levels of	is a marker for					arterial thrombosis	MedicalFinding	activity of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_382_s_154	14656741	27,28  This issue is especially relevant given the fact that plasma gammaA/gamma'' fibrinogen levels are a marker of arterial thrombotic activity, and also given that fibrinogen gamma'' chain displays much less binding to the platelet fibrinogen receptor, glycoprotein IIb/IIa. 17,29  Finally, other issues are the interaction between fibrin architecture and the plasma gammaA/gamma'' fibrinogen level, as well as the factor XIIIa Val34Leu polymorphism, which affects both the physical properties of the fibrin network and platelet deposition in vitro and confers a protective effect on subjects for the occurrence of myocardial infarction.	bind
30146	2	7492	5	13	NULL	NULL	NULL	fibrinogen gamma'' chain	GP		bind		less			glycoprotein IIb/IIa	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_382_s_154	14656741	27,28  This issue is especially relevant given the fact that plasma gammaA/gamma'' fibrinogen levels are a marker of arterial thrombotic activity, and also given that fibrinogen gamma'' chain displays much less binding to the platelet fibrinogen receptor, glycoprotein IIb/IIa. 17,29  Finally, other issues are the interaction between fibrin architecture and the plasma gammaA/gamma'' fibrinogen level, as well as the factor XIIIa Val34Leu polymorphism, which affects both the physical properties of the fibrin network and platelet deposition in vitro and confers a protective effect on subjects for the occurrence of myocardial infarction.	bind
30147	3	7492	5	13	NULL	NULL	NULL	glycoprotein IIb/IIa	GP		is a type of					platelet fibrinogen receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_382_s_154	14656741	27,28  This issue is especially relevant given the fact that plasma gammaA/gamma'' fibrinogen levels are a marker of arterial thrombotic activity, and also given that fibrinogen gamma'' chain displays much less binding to the platelet fibrinogen receptor, glycoprotein IIb/IIa. 17,29  Finally, other issues are the interaction between fibrin architecture and the plasma gammaA/gamma'' fibrinogen level, as well as the factor XIIIa Val34Leu polymorphism, which affects both the physical properties of the fibrin network and platelet deposition in vitro and confers a protective effect on subjects for the occurrence of myocardial infarction.	bind
30148	4	7492	5	13	NULL	NULL	NULL	fibrin 	GP	architecture	interacts with					plasma gammaA/gamma'' fibrinogen	GP	levels of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_382_s_154	14656741	27,28  This issue is especially relevant given the fact that plasma gammaA/gamma'' fibrinogen levels are a marker of arterial thrombotic activity, and also given that fibrinogen gamma'' chain displays much less binding to the platelet fibrinogen receptor, glycoprotein IIb/IIa. 17,29  Finally, other issues are the interaction between fibrin architecture and the plasma gammaA/gamma'' fibrinogen level, as well as the factor XIIIa Val34Leu polymorphism, which affects both the physical properties of the fibrin network and platelet deposition in vitro and confers a protective effect on subjects for the occurrence of myocardial infarction.	bind
30149	5	7492	5	13	NULL	NULL	NULL	fibrin	GP	architecture	interacts with					factor XIIIa polymorphism	GP		Val34Leu		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_382_s_154	14656741	27,28  This issue is especially relevant given the fact that plasma gammaA/gamma'' fibrinogen levels are a marker of arterial thrombotic activity, and also given that fibrinogen gamma'' chain displays much less binding to the platelet fibrinogen receptor, glycoprotein IIb/IIa. 17,29  Finally, other issues are the interaction between fibrin architecture and the plasma gammaA/gamma'' fibrinogen level, as well as the factor XIIIa Val34Leu polymorphism, which affects both the physical properties of the fibrin network and platelet deposition in vitro and confers a protective effect on subjects for the occurrence of myocardial infarction.	bind
30150	6	7492	5	13	NULL	NULL	NULL	statement 4	Process		affects					fibrin network	CellComponent	physical properties of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_382_s_154	14656741	27,28  This issue is especially relevant given the fact that plasma gammaA/gamma'' fibrinogen levels are a marker of arterial thrombotic activity, and also given that fibrinogen gamma'' chain displays much less binding to the platelet fibrinogen receptor, glycoprotein IIb/IIa. 17,29  Finally, other issues are the interaction between fibrin architecture and the plasma gammaA/gamma'' fibrinogen level, as well as the factor XIIIa Val34Leu polymorphism, which affects both the physical properties of the fibrin network and platelet deposition in vitro and confers a protective effect on subjects for the occurrence of myocardial infarction.	bind
30151	7	7492	5	13	NULL	NULL	NULL	statement 5	Process		affects					fibrin network	CellComponent	physical properties of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_382_s_154	14656741	27,28  This issue is especially relevant given the fact that plasma gammaA/gamma'' fibrinogen levels are a marker of arterial thrombotic activity, and also given that fibrinogen gamma'' chain displays much less binding to the platelet fibrinogen receptor, glycoprotein IIb/IIa. 17,29  Finally, other issues are the interaction between fibrin architecture and the plasma gammaA/gamma'' fibrinogen level, as well as the factor XIIIa Val34Leu polymorphism, which affects both the physical properties of the fibrin network and platelet deposition in vitro and confers a protective effect on subjects for the occurrence of myocardial infarction.	bind
30152	8	7492	5	13	NULL	NULL	NULL	statement 4	Process		affects					platelet	Cell	deposition of			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_382_s_154	14656741	27,28  This issue is especially relevant given the fact that plasma gammaA/gamma'' fibrinogen levels are a marker of arterial thrombotic activity, and also given that fibrinogen gamma'' chain displays much less binding to the platelet fibrinogen receptor, glycoprotein IIb/IIa. 17,29  Finally, other issues are the interaction between fibrin architecture and the plasma gammaA/gamma'' fibrinogen level, as well as the factor XIIIa Val34Leu polymorphism, which affects both the physical properties of the fibrin network and platelet deposition in vitro and confers a protective effect on subjects for the occurrence of myocardial infarction.	bind
30153	9	7492	5	13	NULL	NULL	NULL	statement 5	Process		affects					platelet	Cell	deposition of			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_382_s_154	14656741	27,28  This issue is especially relevant given the fact that plasma gammaA/gamma'' fibrinogen levels are a marker of arterial thrombotic activity, and also given that fibrinogen gamma'' chain displays much less binding to the platelet fibrinogen receptor, glycoprotein IIb/IIa. 17,29  Finally, other issues are the interaction between fibrin architecture and the plasma gammaA/gamma'' fibrinogen level, as well as the factor XIIIa Val34Leu polymorphism, which affects both the physical properties of the fibrin network and platelet deposition in vitro and confers a protective effect on subjects for the occurrence of myocardial infarction.	bind
30154	10	7492	5	13	NULL	NULL	NULL	statement 4	Process		confers					myocardial infarction	Process	protective effect on occurrence of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_382_s_154	14656741	27,28  This issue is especially relevant given the fact that plasma gammaA/gamma'' fibrinogen levels are a marker of arterial thrombotic activity, and also given that fibrinogen gamma'' chain displays much less binding to the platelet fibrinogen receptor, glycoprotein IIb/IIa. 17,29  Finally, other issues are the interaction between fibrin architecture and the plasma gammaA/gamma'' fibrinogen level, as well as the factor XIIIa Val34Leu polymorphism, which affects both the physical properties of the fibrin network and platelet deposition in vitro and confers a protective effect on subjects for the occurrence of myocardial infarction.	bind
30155	11	7492	5	13	NULL	NULL	NULL	myocardial infarction	Process		confers					myocardial infarction	Process	protective effect on occurrence of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_382_s_154	14656741	27,28  This issue is especially relevant given the fact that plasma gammaA/gamma'' fibrinogen levels are a marker of arterial thrombotic activity, and also given that fibrinogen gamma'' chain displays much less binding to the platelet fibrinogen receptor, glycoprotein IIb/IIa. 17,29  Finally, other issues are the interaction between fibrin architecture and the plasma gammaA/gamma'' fibrinogen level, as well as the factor XIIIa Val34Leu polymorphism, which affects both the physical properties of the fibrin network and platelet deposition in vitro and confers a protective effect on subjects for the occurrence of myocardial infarction.	bind
30217	1	7492	7	NULL	NULL	0	NULL	fibrinogen	NULL		bind	NULL	less	gamma chain		fibrinogen receptor	NULL	platelet			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_382_s_154	14656741	27,28  This issue is especially relevant given the fact that plasma gammaA/gamma'' fibrinogen levels are a marker of arterial thrombotic activity, and also given that fibrinogen gamma'' chain displays much less binding to the platelet fibrinogen receptor, glycoprotein IIb/IIa. 17,29  Finally, other issues are the interaction between fibrin architecture and the plasma gammaA/gamma'' fibrinogen level, as well as the factor XIIIa Val34Leu polymorphism, which affects both the physical properties of the fibrin network and platelet deposition in vitro and confers a protective effect on subjects for the occurrence of myocardial infarction.	bind
30218	2	7492	7	NULL	NULL	0	NULL	fibrinogen	NULL		bind	NULL	less	gamma chain		glycoprotein IIb/IIa	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_382_s_154	14656741	27,28  This issue is especially relevant given the fact that plasma gammaA/gamma'' fibrinogen levels are a marker of arterial thrombotic activity, and also given that fibrinogen gamma'' chain displays much less binding to the platelet fibrinogen receptor, glycoprotein IIb/IIa. 17,29  Finally, other issues are the interaction between fibrin architecture and the plasma gammaA/gamma'' fibrinogen level, as well as the factor XIIIa Val34Leu polymorphism, which affects both the physical properties of the fibrin network and platelet deposition in vitro and confers a protective effect on subjects for the occurrence of myocardial infarction.	bind
30219	3	7492	7	NULL	NULL	0	NULL	 gammaA/gamma'' fibrinogen levels	NULL	plasma	is a marker of	NULL				arterial thrombotic activity	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_382_s_154	14656741	27,28  This issue is especially relevant given the fact that plasma gammaA/gamma'' fibrinogen levels are a marker of arterial thrombotic activity, and also given that fibrinogen gamma'' chain displays much less binding to the platelet fibrinogen receptor, glycoprotein IIb/IIa. 17,29  Finally, other issues are the interaction between fibrin architecture and the plasma gammaA/gamma'' fibrinogen level, as well as the factor XIIIa Val34Leu polymorphism, which affects both the physical properties of the fibrin network and platelet deposition in vitro and confers a protective effect on subjects for the occurrence of myocardial infarction.	bind
30220	4	7492	7	NULL	NULL	0	NULL	fibrin architecture	NULL	interaction between	affect	NULL				fibrin network	NULL	physical property of			NULL	in vitro	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_382_s_154	14656741	27,28  This issue is especially relevant given the fact that plasma gammaA/gamma'' fibrinogen levels are a marker of arterial thrombotic activity, and also given that fibrinogen gamma'' chain displays much less binding to the platelet fibrinogen receptor, glycoprotein IIb/IIa. 17,29  Finally, other issues are the interaction between fibrin architecture and the plasma gammaA/gamma'' fibrinogen level, as well as the factor XIIIa Val34Leu polymorphism, which affects both the physical properties of the fibrin network and platelet deposition in vitro and confers a protective effect on subjects for the occurrence of myocardial infarction.	bind
30221	5	7492	7	NULL	NULL	0	NULL	gammaA/gamma'' fibrinogen level	NULL	plasma	affect	NULL				fibrin network	NULL	physical property of			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_382_s_154	14656741	27,28  This issue is especially relevant given the fact that plasma gammaA/gamma'' fibrinogen levels are a marker of arterial thrombotic activity, and also given that fibrinogen gamma'' chain displays much less binding to the platelet fibrinogen receptor, glycoprotein IIb/IIa. 17,29  Finally, other issues are the interaction between fibrin architecture and the plasma gammaA/gamma'' fibrinogen level, as well as the factor XIIIa Val34Leu polymorphism, which affects both the physical properties of the fibrin network and platelet deposition in vitro and confers a protective effect on subjects for the occurrence of myocardial infarction.	bind
30222	6	7492	7	NULL	NULL	0	NULL	factor XIIIa	NULL	polymorphic	affect	NULL		Val34Leu		fibrin network	NULL	physical property of			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_382_s_154	14656741	27,28  This issue is especially relevant given the fact that plasma gammaA/gamma'' fibrinogen levels are a marker of arterial thrombotic activity, and also given that fibrinogen gamma'' chain displays much less binding to the platelet fibrinogen receptor, glycoprotein IIb/IIa. 17,29  Finally, other issues are the interaction between fibrin architecture and the plasma gammaA/gamma'' fibrinogen level, as well as the factor XIIIa Val34Leu polymorphism, which affects both the physical properties of the fibrin network and platelet deposition in vitro and confers a protective effect on subjects for the occurrence of myocardial infarction.	bind
30223	7	7492	7	NULL	NULL	0	NULL	fibrin architecture	NULL	interaction between	affect	NULL				platelet deposition	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_382_s_154	14656741	27,28  This issue is especially relevant given the fact that plasma gammaA/gamma'' fibrinogen levels are a marker of arterial thrombotic activity, and also given that fibrinogen gamma'' chain displays much less binding to the platelet fibrinogen receptor, glycoprotein IIb/IIa. 17,29  Finally, other issues are the interaction between fibrin architecture and the plasma gammaA/gamma'' fibrinogen level, as well as the factor XIIIa Val34Leu polymorphism, which affects both the physical properties of the fibrin network and platelet deposition in vitro and confers a protective effect on subjects for the occurrence of myocardial infarction.	bind
30224	8	7492	7	NULL	NULL	0	NULL	 gammaA/gamma'' fibrinogen level	NULL	plasma	affect	NULL				platelet deposition	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_382_s_154	14656741	27,28  This issue is especially relevant given the fact that plasma gammaA/gamma'' fibrinogen levels are a marker of arterial thrombotic activity, and also given that fibrinogen gamma'' chain displays much less binding to the platelet fibrinogen receptor, glycoprotein IIb/IIa. 17,29  Finally, other issues are the interaction between fibrin architecture and the plasma gammaA/gamma'' fibrinogen level, as well as the factor XIIIa Val34Leu polymorphism, which affects both the physical properties of the fibrin network and platelet deposition in vitro and confers a protective effect on subjects for the occurrence of myocardial infarction.	bind
30225	9	7492	7	NULL	NULL	0	NULL	factor XIIIa	NULL	polymorphic	affect	NULL		Val34Leu		platelet deposition	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_382_s_154	14656741	27,28  This issue is especially relevant given the fact that plasma gammaA/gamma'' fibrinogen levels are a marker of arterial thrombotic activity, and also given that fibrinogen gamma'' chain displays much less binding to the platelet fibrinogen receptor, glycoprotein IIb/IIa. 17,29  Finally, other issues are the interaction between fibrin architecture and the plasma gammaA/gamma'' fibrinogen level, as well as the factor XIIIa Val34Leu polymorphism, which affects both the physical properties of the fibrin network and platelet deposition in vitro and confers a protective effect on subjects for the occurrence of myocardial infarction.	bind
30226	10	7492	7	NULL	NULL	0	NULL	fibrin architecture	NULL	interaction between	effect	NULL				myocardial infarction	NULL	the occurence of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_382_s_154	14656741	27,28  This issue is especially relevant given the fact that plasma gammaA/gamma'' fibrinogen levels are a marker of arterial thrombotic activity, and also given that fibrinogen gamma'' chain displays much less binding to the platelet fibrinogen receptor, glycoprotein IIb/IIa. 17,29  Finally, other issues are the interaction between fibrin architecture and the plasma gammaA/gamma'' fibrinogen level, as well as the factor XIIIa Val34Leu polymorphism, which affects both the physical properties of the fibrin network and platelet deposition in vitro and confers a protective effect on subjects for the occurrence of myocardial infarction.	bind
30227	11	7492	7	NULL	NULL	0	NULL	gammaA/gamma'' fibrinogen level	NULL	plasma	effect	NULL				myocardial infarction	NULL	the occurence of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_382_s_154	14656741	27,28  This issue is especially relevant given the fact that plasma gammaA/gamma'' fibrinogen levels are a marker of arterial thrombotic activity, and also given that fibrinogen gamma'' chain displays much less binding to the platelet fibrinogen receptor, glycoprotein IIb/IIa. 17,29  Finally, other issues are the interaction between fibrin architecture and the plasma gammaA/gamma'' fibrinogen level, as well as the factor XIIIa Val34Leu polymorphism, which affects both the physical properties of the fibrin network and platelet deposition in vitro and confers a protective effect on subjects for the occurrence of myocardial infarction.	bind
30228	12	7492	7	NULL	NULL	0	NULL	factor XIIIa	NULL	polymorphic	effect	NULL		Val34Leu		myocardial infarction	NULL	occurence of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_382_s_154	14656741	27,28  This issue is especially relevant given the fact that plasma gammaA/gamma'' fibrinogen levels are a marker of arterial thrombotic activity, and also given that fibrinogen gamma'' chain displays much less binding to the platelet fibrinogen receptor, glycoprotein IIb/IIa. 17,29  Finally, other issues are the interaction between fibrin architecture and the plasma gammaA/gamma'' fibrinogen level, as well as the factor XIIIa Val34Leu polymorphism, which affects both the physical properties of the fibrin network and platelet deposition in vitro and confers a protective effect on subjects for the occurrence of myocardial infarction.	bind
28172	1	7493	5	13	NULL	NULL	NULL	TIMPs	GP	activated	bind					MMPs	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_4_716_s_83	16469948	27,28  TIMPs bind activated MMPs to form equimolar complexes.	bind
28173	2	7493	5	13	NULL	NULL	NULL	statement 1	Process		forms					equimolar complexes	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_4_716_s_83	16469948	27,28  TIMPs bind activated MMPs to form equimolar complexes.	bind
30229	1	7493	7	NULL	NULL	0	NULL	TIMPs	NULL		bind	NULL				MMPs	NULL	activated			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_4_716_s_83	16469948	27,28  TIMPs bind activated MMPs to form equimolar complexes.	bind
30230	2	7493	7	NULL	NULL	0	NULL	statement 1	NULL		form	NULL				equimolar complexes	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_4_716_s_83	16469948	27,28  TIMPs bind activated MMPs to form equimolar complexes.	bind
28174	1	7494	5	13	NULL	NULL	NULL	VH4-34 gene	GP		is found in		virtually			cold agglutinin disease	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_253_s_160	11438472	27- 32  Interestingly, the  VH4-34 gene is found in virtually all cases of cold agglutinin disease 33- 35 and the red blood cell I/i antigens bind to the FR1 domain of Ig.	bind
28175	2	7494	5	13	NULL	NULL	NULL	I/i antigens	Chemical	red blood cell	bind					Ig	GP		FR1 domain		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_253_s_160	11438472	27- 32  Interestingly, the  VH4-34 gene is found in virtually all cases of cold agglutinin disease 33- 35 and the red blood cell I/i antigens bind to the FR1 domain of Ig.	bind
30231	1	7494	7	NULL	NULL	0	NULL	VH4-34 gene	NULL		is found in	NULL				cold agglutinin disease	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_1_253_s_160	11438472	27- 32  Interestingly, the  VH4-34 gene is found in virtually all cases of cold agglutinin disease 33- 35 and the red blood cell I/i antigens bind to the FR1 domain of Ig.	bind
30232	2	7494	7	NULL	NULL	0	NULL	 I/i antigens	NULL	 red blood cell 	bind	NULL				Ig	NULL		FR1 domain		NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_1_253_s_160	11438472	27- 32  Interestingly, the  VH4-34 gene is found in virtually all cases of cold agglutinin disease 33- 35 and the red blood cell I/i antigens bind to the FR1 domain of Ig.	bind
28176	1	7495	5	13	NULL	NULL	NULL	Poly (rC) binding protein 2	GP		forms a ternary complex with					poliovirus RNA	NucleicAcid		5''- terminal sequences		NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_11_2427_s_399	11376162	28       Parsley,T.B., Towner,J.S., Blyn,L.B., Ehrenfeld,E. and Semler,B.L. (1997) Poly (rC) binding protein 2 forms a ternary complex with the 5''- terminal sequences of poliovirus RNA and the viral 3CD proteinase .	bind
28177	2	7495	5	13	NULL	NULL	NULL	Poly (rC) binding protein 2	GP		forms a ternary complex with					viral 3CD proteinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_11_2427_s_399	11376162	28       Parsley,T.B., Towner,J.S., Blyn,L.B., Ehrenfeld,E. and Semler,B.L. (1997) Poly (rC) binding protein 2 forms a ternary complex with the 5''- terminal sequences of poliovirus RNA and the viral 3CD proteinase .	bind
30233	1	7495	7	NULL	NULL	0	NULL	Poly (rC) binding protein 2	NULL		forms a ternary complex with	NULL				poliovirus RNA	NULL		 5''- terminal sequences of		NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_11_2427_s_399	11376162	28       Parsley,T.B., Towner,J.S., Blyn,L.B., Ehrenfeld,E. and Semler,B.L. (1997) Poly (rC) binding protein 2 forms a ternary complex with the 5''- terminal sequences of poliovirus RNA and the viral 3CD proteinase .	bind
30234	2	7495	7	NULL	NULL	0	NULL	Poly (rC) binding protein 2	NULL		forms a ternary complex with	NULL				viral 3CD proteinase	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_11_2427_s_399	11376162	28       Parsley,T.B., Towner,J.S., Blyn,L.B., Ehrenfeld,E. and Semler,B.L. (1997) Poly (rC) binding protein 2 forms a ternary complex with the 5''- terminal sequences of poliovirus RNA and the viral 3CD proteinase .	bind
28178	1	7496	5	13	NULL	NULL	NULL	Flt-1	GP		undergoes					phosphorylation	Process	minimal	tyrosine		NULL	transfected cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_5_765_s_128	11348872	28  Flt-1 shows minimal tyrosine phosphorylation in response to VEGF, and binding of VEGF does not lead to significant biological roles in transfected cells.	bind
28179	2	7496	5	13	NULL	NULL	NULL	statement 1	Process		occurs in response to					VEGF	GP				NULL	transfected cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_5_765_s_128	11348872	28  Flt-1 shows minimal tyrosine phosphorylation in response to VEGF, and binding of VEGF does not lead to significant biological roles in transfected cells.	bind
28180	3	7496	5	13	NULL	NULL	NULL	VEGF	GP	binding of	does not lead to					biological roles	Process	significant			NULL	in transfected cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_5_765_s_128	11348872	28  Flt-1 shows minimal tyrosine phosphorylation in response to VEGF, and binding of VEGF does not lead to significant biological roles in transfected cells.	bind
30235	1	7496	7	10	NULL	0	NULL	Flt-1	NULL		undergoes	NULL				phosphorylation	NULL	minimal	tyrosine		NULL	transfected cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_5_765_s_128	11348872	28  Flt-1 shows minimal tyrosine phosphorylation in response to VEGF, and binding of VEGF does not lead to significant biological roles in transfected cells.	bind
30236	2	7496	7	NULL	NULL	0	NULL	statement 1	NULL		in response to	NULL				VEGF	NULL				NULL	transfected cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_5_765_s_128	11348872	28  Flt-1 shows minimal tyrosine phosphorylation in response to VEGF, and binding of VEGF does not lead to significant biological roles in transfected cells.	bind
30237	3	7496	7	NULL	NULL	0	NULL	Flt-1	NULL		bind	NULL				VEGF	NULL				NULL	transfected cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_5_765_s_128	11348872	28  Flt-1 shows minimal tyrosine phosphorylation in response to VEGF, and binding of VEGF does not lead to significant biological roles in transfected cells.	bind
30238	4	7496	7	NULL	NULL	0	NULL	statement 3	NULL		does not lead to	NULL				biological role	NULL	significant			NULL	transfected cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_5_765_s_128	11348872	28  Flt-1 shows minimal tyrosine phosphorylation in response to VEGF, and binding of VEGF does not lead to significant biological roles in transfected cells.	bind
28181	1	7497	5	13	NULL	NULL	NULL	insulin	GP		causes					smooth muscle cell	Cell	proliferation of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulation_91_3_831_s_180	7828312	28  In vitro, insulin has been shown to cause smooth muscle cell proliferation 29 ; stimulate LDL binding to smooth muscle cells, 30  fibroblasts, 31  and monocytes 32 ; and stimulate cholesterol synthesis in monocytes.	bind
28182	2	7497	5	13	NULL	NULL	NULL	LDL	GP		bind					smooth muscle cells	Cell				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulation_91_3_831_s_180	7828312	28  In vitro, insulin has been shown to cause smooth muscle cell proliferation 29 ; stimulate LDL binding to smooth muscle cells, 30  fibroblasts, 31  and monocytes 32 ; and stimulate cholesterol synthesis in monocytes.	bind
28183	3	7497	5	13	NULL	NULL	NULL	insulin	GP		stimulates					statement 2	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulation_91_3_831_s_180	7828312	28  In vitro, insulin has been shown to cause smooth muscle cell proliferation 29 ; stimulate LDL binding to smooth muscle cells, 30  fibroblasts, 31  and monocytes 32 ; and stimulate cholesterol synthesis in monocytes.	bind
28184	4	7497	5	13	NULL	NULL	NULL	LDL	GP		bind					fibroblasts	Cell				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulation_91_3_831_s_180	7828312	28  In vitro, insulin has been shown to cause smooth muscle cell proliferation 29 ; stimulate LDL binding to smooth muscle cells, 30  fibroblasts, 31  and monocytes 32 ; and stimulate cholesterol synthesis in monocytes.	bind
28185	5	7497	5	13	NULL	NULL	NULL	insulin	GP		stimulates					statement 4	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulation_91_3_831_s_180	7828312	28  In vitro, insulin has been shown to cause smooth muscle cell proliferation 29 ; stimulate LDL binding to smooth muscle cells, 30  fibroblasts, 31  and monocytes 32 ; and stimulate cholesterol synthesis in monocytes.	bind
28186	6	7497	5	13	NULL	NULL	NULL	LDL	GP		bind					monocytes	Cell				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulation_91_3_831_s_180	7828312	28  In vitro, insulin has been shown to cause smooth muscle cell proliferation 29 ; stimulate LDL binding to smooth muscle cells, 30  fibroblasts, 31  and monocytes 32 ; and stimulate cholesterol synthesis in monocytes.	bind
28187	7	7497	5	13	NULL	NULL	NULL	insulin	GP		stimulates					statement 6	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulation_91_3_831_s_180	7828312	28  In vitro, insulin has been shown to cause smooth muscle cell proliferation 29 ; stimulate LDL binding to smooth muscle cells, 30  fibroblasts, 31  and monocytes 32 ; and stimulate cholesterol synthesis in monocytes.	bind
28188	7	7497	5	13	NULL	NULL	NULL	insulin	GP		stimulates					statement 6	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulation_91_3_831_s_180	7828312	28  In vitro, insulin has been shown to cause smooth muscle cell proliferation 29 ; stimulate LDL binding to smooth muscle cells, 30  fibroblasts, 31  and monocytes 32 ; and stimulate cholesterol synthesis in monocytes.	bind
28189	8	7497	5	13	NULL	NULL	NULL	insulin	GP		stimulates					cholesterol	Chemical	synthesis of			NULL	in vitro, in monocytes	NULL	NULL	NULL	NULL	gw60_circulation_91_3_831_s_180	7828312	28  In vitro, insulin has been shown to cause smooth muscle cell proliferation 29 ; stimulate LDL binding to smooth muscle cells, 30  fibroblasts, 31  and monocytes 32 ; and stimulate cholesterol synthesis in monocytes.	bind
30239	1	7497	7	NULL	NULL	0	NULL	insulin	NULL		cause	NULL				smooth muscle cell proliferation	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_circulation_91_3_831_s_180	7828312	28  In vitro, insulin has been shown to cause smooth muscle cell proliferation 29 ; stimulate LDL binding to smooth muscle cells, 30  fibroblasts, 31  and monocytes 32 ; and stimulate cholesterol synthesis in monocytes.	bind
30240	2	7497	7	NULL	NULL	0	NULL	LDL	NULL		bind	NULL				smooth muscle cells	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulation_91_3_831_s_180	7828312	28  In vitro, insulin has been shown to cause smooth muscle cell proliferation 29 ; stimulate LDL binding to smooth muscle cells, 30  fibroblasts, 31  and monocytes 32 ; and stimulate cholesterol synthesis in monocytes.	bind
30241	3	7497	7	NULL	NULL	0	NULL	LDL	NULL		bind	NULL				fibroblasts	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_circulation_91_3_831_s_180	7828312	28  In vitro, insulin has been shown to cause smooth muscle cell proliferation 29 ; stimulate LDL binding to smooth muscle cells, 30  fibroblasts, 31  and monocytes 32 ; and stimulate cholesterol synthesis in monocytes.	bind
30242	4	7497	7	NULL	NULL	0	NULL	LDL	NULL		bind	NULL				monocytes	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulation_91_3_831_s_180	7828312	28  In vitro, insulin has been shown to cause smooth muscle cell proliferation 29 ; stimulate LDL binding to smooth muscle cells, 30  fibroblasts, 31  and monocytes 32 ; and stimulate cholesterol synthesis in monocytes.	bind
30243	5	7497	7	NULL	NULL	0	NULL	insulin	NULL		stimulate	NULL				statement 2	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_circulation_91_3_831_s_180	7828312	28  In vitro, insulin has been shown to cause smooth muscle cell proliferation 29 ; stimulate LDL binding to smooth muscle cells, 30  fibroblasts, 31  and monocytes 32 ; and stimulate cholesterol synthesis in monocytes.	bind
30244	6	7497	7	NULL	NULL	0	NULL	insulin	NULL		stimulate	NULL				statement 3	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_circulation_91_3_831_s_180	7828312	28  In vitro, insulin has been shown to cause smooth muscle cell proliferation 29 ; stimulate LDL binding to smooth muscle cells, 30  fibroblasts, 31  and monocytes 32 ; and stimulate cholesterol synthesis in monocytes.	bind
30245	7	7497	7	NULL	NULL	0	NULL	insulin	NULL		stimulate	NULL				statement 4	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulation_91_3_831_s_180	7828312	28  In vitro, insulin has been shown to cause smooth muscle cell proliferation 29 ; stimulate LDL binding to smooth muscle cells, 30  fibroblasts, 31  and monocytes 32 ; and stimulate cholesterol synthesis in monocytes.	bind
30246	8	7497	7	10	NULL	0	NULL	insulin			stimulate					cholesterol		synthesis of			NULL	monocytes, in vitro	NULL	NULL	NULL	NULL	gw60_circulation_91_3_831_s_180	7828312	28  In vitro, insulin has been shown to cause smooth muscle cell proliferation 29 ; stimulate LDL binding to smooth muscle cells, 30  fibroblasts, 31  and monocytes 32 ; and stimulate cholesterol synthesis in monocytes.	bind
28225	1	7498	5	13	NULL	NULL	NULL	activator protein-1	GP		bind									DNA binding sites	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_1_244_s_197	10634825	28  Our previous study showed that lysoPC was capable of stimulating the binding of activator protein-1 and nuclear factor-kappaB to the DNA binding sites.	bind
28226	2	7498	5	13	NULL	NULL	NULL	nuclear factor-kappaB	GP		bind									DNA binding sites	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_1_244_s_197	10634825	28  Our previous study showed that lysoPC was capable of stimulating the binding of activator protein-1 and nuclear factor-kappaB to the DNA binding sites.	bind
28227	3	7498	5	13	NULL	NULL	NULL	lysoPC	Chemical		stimulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_1_244_s_197	10634825	28  Our previous study showed that lysoPC was capable of stimulating the binding of activator protein-1 and nuclear factor-kappaB to the DNA binding sites.	bind
28228	4	7498	5	13	NULL	NULL	NULL	lysoPC	Chemical		stimulates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_1_244_s_197	10634825	28  Our previous study showed that lysoPC was capable of stimulating the binding of activator protein-1 and nuclear factor-kappaB to the DNA binding sites.	bind
30247	1	7498	7	10	NULL	0	NULL	activator protein-1			bind									DNA binding site	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_1_244_s_197	10634825	28  Our previous study showed that lysoPC was capable of stimulating the binding of activator protein-1 and nuclear factor-kappaB to the DNA binding sites.	bind
30248	2	7498	7	10	NULL	0	NULL	nuclear factor-kappaB			bind									DNA binding site	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_1_244_s_197	10634825	28  Our previous study showed that lysoPC was capable of stimulating the binding of activator protein-1 and nuclear factor-kappaB to the DNA binding sites.	bind
30249	3	7498	7	NULL	NULL	0	NULL	 lysoPC	NULL		stimulate	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_1_244_s_197	10634825	28  Our previous study showed that lysoPC was capable of stimulating the binding of activator protein-1 and nuclear factor-kappaB to the DNA binding sites.	bind
30250	4	7498	7	NULL	NULL	0	NULL	lysoPC	NULL		stimulate	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_1_244_s_197	10634825	28  Our previous study showed that lysoPC was capable of stimulating the binding of activator protein-1 and nuclear factor-kappaB to the DNA binding sites.	bind
28223	1	7499	5	13	NULL	NULL	NULL	proteins	GP	extracted from HTC rat hepatoma cells	bind					Sp1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_12_2696_s_184	11116074	28  Proteins extracted from HTC rat hepatoma cells bind to Sp1 and CTF/NF-1 - like binding sites in the rat PAI-1 regulatory region.	bind
28224	2	7499	5	13	NULL	NULL	NULL	proteins	GP	extracted from HTC rat hepatoma cells	bind					PAI-1	GP	rat		CTF/NF-1 - like binding sites in regulatory region	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_12_2696_s_184	11116074	28  Proteins extracted from HTC rat hepatoma cells bind to Sp1 and CTF/NF-1 - like binding sites in the rat PAI-1 regulatory region.	bind
30251	1	7499	7	NULL	NULL	0	NULL	hepatoma cells	NULL	HTC rat	bind	NULL				 Sp1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_12_2696_s_184	11116074	28  Proteins extracted from HTC rat hepatoma cells bind to Sp1 and CTF/NF-1 - like binding sites in the rat PAI-1 regulatory region.	bind
30252	2	7499	7	NULL	NULL	0	NULL	hepatoma cells	NULL	HTC rat	bind	NULL				PAI-1	NULL	rat		CTF/NF-1 - like binding sites in the regulatory region	NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_12_2696_s_184	11116074	28  Proteins extracted from HTC rat hepatoma cells bind to Sp1 and CTF/NF-1 - like binding sites in the rat PAI-1 regulatory region.	bind
28203	1	7500	5	13	NULL	NULL	NULL	endothelial cell growth factor	GP		bind					FGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_1_178_s_203	9888881	28  Similar observations have been made by Nanberg et al 29  for another endothelial cell growth factor which binds to a tyrosine kinase receptor, namely FGF.	bind
28209	2	7500	5	13	NULL	NULL	NULL	FGF	GP		is a type of					tyrosine kinase receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_1_178_s_203	9888881	28  Similar observations have been made by Nanberg et al 29  for another endothelial cell growth factor which binds to a tyrosine kinase receptor, namely FGF.	bind
30253	1	7500	7	NULL	NULL	0	NULL	endothelial cell growth factor	NULL		binds	NULL				FGF	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_1_178_s_203	9888881	28  Similar observations have been made by Nanberg et al 29  for another endothelial cell growth factor which binds to a tyrosine kinase receptor, namely FGF.	bind
30254	2	7500	7	NULL	NULL	0	NULL	FGF	NULL		is a type of	NULL				tyrosine kinase receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_1_178_s_203	9888881	28  Similar observations have been made by Nanberg et al 29  for another endothelial cell growth factor which binds to a tyrosine kinase receptor, namely FGF.	bind
29869	1	7502	5	13	NULL	NULL	NULL	apoE	GP	neuronal	bind		may;;potentially			Abeta	GP				NULL	intraneuronally	NULL	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
29870	2	7502	5	13	NULL	NULL	NULL	apoE	GP	astrocyte-generated	bind		may;;potentially			Abeta	GP				NULL	intraneuronally	NULL	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
29872	3	7502	5	13	NULL	NULL	NULL	apoE	GP	neuronal	bind		may;;potentially			Abeta	GP				NULL	extracellularly 	NULL	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
29874	4	7502	5	13	NULL	NULL	NULL	apoE	GP	astrocyte-generated	bind		may;;potentially			Abeta	GP				NULL	extracellularly	NULL	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
29876	5	7502	5	13	NULL	NULL	NULL	statement 1	Process		leads to					neurons	Cell	internalization of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
29880	6	7502	5	13	NULL	NULL	NULL	statement 2	Process		leads to					neurons	Cell	internalization of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
29881	7	7502	5	13	NULL	NULL	NULL	statement 3	Process		leads to					neurons	Cell	internalization of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
29882	8	7502	5	13	NULL	NULL	NULL	statement 4	Process		leads to					neurons	Cell	internalization of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
29883	9	7502	5	13	NULL	NULL	NULL	Abeta	GP	accumulation of	leads to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
29885	10	7502	5	13	NULL	NULL	NULL	Abeta	GP	accumulation of	leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
29886	11	7502	5	13	NULL	NULL	NULL	Abeta	GP	accumulation of	leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
29887	12	7502	5	13	NULL	NULL	NULL	Abeta	GP	accumulation of	leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
29889	13	7502	5	13	NULL	NULL	NULL	neuronal dysfunction	MedicalFinding		leads to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
29890	14	7502	5	13	NULL	NULL	NULL	neuronal dysfunction	MedicalFinding		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
29892	18	7502	5	13	NULL	NULL	NULL	apoE	GP	increased immunoreactivity of	is observed in					statement 17	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
54522	15	7502	5	13	NULL	NULL	NULL	neuronal dysfunction	MedicalFinding		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
54523	16	7502	5	13	NULL	NULL	NULL	neuronal dysfunction	MedicalFinding		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
54524	17	7502	5	13	NULL	NULL	NULL	neurons	Cell		immunoreactive to					Abeta42	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
30481	1	7502	7	NULL	NULL	0	NULL	apoE	NULL	neuronal	bind	NULL	may;;potentially			Abeta	NULL				NULL	intraneuronal	NULL	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
30482	2	7502	7	NULL	NULL	0	NULL	apoE	NULL	astrocyte-generated 	bind	NULL	may;;potentially			Abeta	NULL				NULL	intraneuronal	NULL	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
30483	3	7502	7	NULL	NULL	0	NULL	apoE	NULL	neuronal	bind	NULL	may;;potentially			Abeta	NULL				NULL	extracellular	0	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
30484	4	7502	7	NULL	NULL	0	NULL	apoE	NULL	astrocyte-generated 	bind	NULL	may;;potentially			Abeta	NULL				NULL	extracellular	0	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
30485	5	7502	7	10	NULL	0	NULL	statement 1			leads to					neurons		internalization of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
30486	6	7502	7	10	NULL	0	NULL	statement 2			leads to					neurons		internalization of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
30487	7	7502	7	10	NULL	0	NULL	statement 3			leads to					neurons		internalization of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
30488	8	7502	7	10	NULL	0	NULL	statement 4			leads to					neurons		internalization of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
30489	9	7502	7	NULL	NULL	0	NULL	statement 1	NULL		occurs with	NULL				Abeta	NULL	accumulation of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
30490	10	7502	7	NULL	NULL	0	NULL	statement 2	NULL		occurs with	NULL				Abeta	NULL	accumulation of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
30491	11	7502	7	NULL	NULL	0	NULL	statement 3	NULL		occurs with	NULL				Abeta	NULL	accumulation of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
30492	12	7502	7	NULL	NULL	0	NULL	statement 4	NULL		occurs with	NULL				Abeta	NULL	accumulation of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
30493	13	7502	7	NULL	NULL	0	NULL	statement 1	NULL		occurs upon	NULL				neuronal dysfunction	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
30494	14	7502	7	NULL	NULL	0	NULL	statement 2	NULL		occurs upon	NULL				neuronal dysfunction	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
30495	15	7502	7	NULL	NULL	0	NULL	statement 3	NULL		occurs upon	NULL				neuronal dysfunction	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
30496	16	7502	7	NULL	NULL	0	NULL	statement 4	NULL		occurs upon	NULL				neuronal dysfunction	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
30497	17	7502	7	10	NULL	0	NULL	neurons			immunoreactive to					Abeta42					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
54525	18	7502	7	10	NULL	0	NULL	apoE		increased immunoreactivity of	is observed in					statement 17					NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_1_15_s_159	10623648	28  With Abeta accumulation and neuronal dysfunction, neuronal or astrocyte-generated apoE may potentially bind to Abeta intraneuronally and/or extracellularly with subsequent neuronal internalization, explaining the observation of apparent increased apoE immunoreactivity in Abeta42 immunoreactive neurons.	bind
28229	1	7503	5	13	NULL	NULL	NULL	HB-EGF	GP		bind					EGFR	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_94_11_2778_s_27	8941102	28 29 30  When HB-EGF binds to an EGFR, it induces EGFR autophosphorylation and exerts various biological activities such as cell proliferation and migration.	bind
28230	2	7503	5	13	NULL	NULL	NULL	statement 1	Process		induces					EGFR	GP	autophosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_94_11_2778_s_27	8941102	28 29 30  When HB-EGF binds to an EGFR, it induces EGFR autophosphorylation and exerts various biological activities such as cell proliferation and migration.	bind
28231	3	7503	5	13	NULL	NULL	NULL	statement 1	Process		exerts					cell proliferation	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_94_11_2778_s_27	8941102	28 29 30  When HB-EGF binds to an EGFR, it induces EGFR autophosphorylation and exerts various biological activities such as cell proliferation and migration.	bind
28232	4	7503	5	13	NULL	NULL	NULL	statement 1	Process		exerts					cell migration	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_94_11_2778_s_27	8941102	28 29 30  When HB-EGF binds to an EGFR, it induces EGFR autophosphorylation and exerts various biological activities such as cell proliferation and migration.	bind
30498	1	7503	7	NULL	NULL	0	NULL	HB-EGF	NULL		binds	NULL				EGFR	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_94_11_2778_s_27	8941102	28 29 30  When HB-EGF binds to an EGFR, it induces EGFR autophosphorylation and exerts various biological activities such as cell proliferation and migration.	bind
30499	2	7503	7	NULL	NULL	0	NULL	statement 1	NULL		induces	NULL				EGFR	NULL	autophosphorylation of			NULL		0	NULL	NULL	NULL	gw60_circulation_94_11_2778_s_27	8941102	28 29 30  When HB-EGF binds to an EGFR, it induces EGFR autophosphorylation and exerts various biological activities such as cell proliferation and migration.	bind
30500	3	7503	7	NULL	NULL	0	NULL	statement 2	NULL		exerts	NULL				cell proliferation	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_94_11_2778_s_27	8941102	28 29 30  When HB-EGF binds to an EGFR, it induces EGFR autophosphorylation and exerts various biological activities such as cell proliferation and migration.	bind
30501	4	7503	7	NULL	NULL	0	NULL	statement 2	NULL		exerts	NULL				cell migration	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_94_11_2778_s_27	8941102	28 29 30  When HB-EGF binds to an EGFR, it induces EGFR autophosphorylation and exerts various biological activities such as cell proliferation and migration.	bind
28233	1	7506	5	13	NULL	NULL	NULL	Ang-4	GP		bind					Tie-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_7_664_s_37	12958144	28 Ang-4 binds to Tie-2 as an agonist, although its precise function has not been documented.	bind
28234	2	7506	5	13	NULL	NULL	NULL	Ang-4	GP		is an agonist of					Tie-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_7_664_s_37	12958144	28 Ang-4 binds to Tie-2 as an agonist, although its precise function has not been documented.	bind
30502	1	7506	7	NULL	NULL	0	NULL	Ang-4	NULL		binds to	NULL				Tie-2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_93_7_664_s_37	12958144	28 Ang-4 binds to Tie-2 as an agonist, although its precise function has not been documented.	bind
30503	2	7506	7	10	NULL	0	NULL	Ang-4			is an agonist of					Tie-2					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_7_664_s_37	12958144	28 Ang-4 binds to Tie-2 as an agonist, although its precise function has not been documented.	bind
28235	1	7507	5	13	NULL	NULL	NULL	Src	GP		bind		weakly			Fak	GP				NULL	in the myocardium of control rats	NULL	NULL	NULL	NULL	gw70_circulationres_96_1_73_s_89	15576648	28 Coimmunoprecipitation assays with anti-Fak and anti-c-Src antibodies showed only a weak binding of Src to Fak in the myocardium of control rats ( Figure 1D and 1E).	bind
30504	1	7507	7	NULL	NULL	0	NULL	Src	NULL		binds	NULL	weakly			Fak	NULL				NULL	myocardium of  rats	0	NULL	NULL	NULL	gw70_circulationres_96_1_73_s_89	15576648	28 Coimmunoprecipitation assays with anti-Fak and anti-c-Src antibodies showed only a weak binding of Src to Fak in the myocardium of control rats ( Figure 1D and 1E).	bind
28236	1	7508	5	13	NULL	NULL	NULL	PTX3	GP		bind					leukemia Jurkat T cells	Cell	human			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_5_782_s_152	12006390	28 Recently, it has been reported that PTX3 binds to human leukemia Jurkat T cells.	bind
30505	1	7508	7	NULL	NULL	0	NULL	PTX3	NULL		binds to	NULL				leukemia Jurkat T cells	NULL	human 			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_5_782_s_152	12006390	28 Recently, it has been reported that PTX3 binds to human leukemia Jurkat T cells.	bind
28237	1	7509	5	13	NULL	NULL	NULL	cGMP	Chemical	receptor-generated	bind					cGK	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_109_2_269_s_171	14718400	28 Receptor-generated cGMP binds to cGK, which is thought to mediate the principal biological functions of cGMP.	bind
28238	2	7509	5	13	NULL	NULL	NULL	statement 1	Process		mediate					cGMP	Chemical	biological functions of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_109_2_269_s_171	14718400	28 Receptor-generated cGMP binds to cGK, which is thought to mediate the principal biological functions of cGMP.	bind
30506	1	7509	7	NULL	NULL	0	NULL	cGMP	NULL	 Receptor-generated	binds	NULL				cGK	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_109_2_269_s_171	14718400	28 Receptor-generated cGMP binds to cGK, which is thought to mediate the principal biological functions of cGMP.	bind
30507	2	7509	7	NULL	NULL	0	NULL	cGK	NULL		mediates	NULL				cGMP	NULL	biological functions of			NULL		0	NULL	NULL	NULL	gw70_circulation_109_2_269_s_171	14718400	28 Receptor-generated cGMP binds to cGK, which is thought to mediate the principal biological functions of cGMP.	bind
28239	1	7510	5	13	NULL	NULL	NULL	synaptotagmin	GP		bind			C2B domain		phosphoinositides	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1152_s_77	12738684	28 The C2B domain of synaptotagmin binds PIP2 preferentially to other phosphoinositides after exposure to Ca2+.	bind
28240	2	7510	5	13	NULL	NULL	NULL	synaptotagmin	GP		bind			C2B domain		PIP2	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1152_s_77	12738684	28 The C2B domain of synaptotagmin binds PIP2 preferentially to other phosphoinositides after exposure to Ca2+.	bind
28241	3	7510	5	13	NULL	NULL	NULL	statement 1	Process		is preferred over					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1152_s_77	12738684	28 The C2B domain of synaptotagmin binds PIP2 preferentially to other phosphoinositides after exposure to Ca2+.	bind
46673	4	7510	5	13	NULL	NULL	NULL	statement 4	Process		occurs after					Ca2+	Chemical	exposure to			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1152_s_77	12738684	28 The C2B domain of synaptotagmin binds PIP2 preferentially to other phosphoinositides after exposure to Ca2+.	bind
30508	1	7510	7	10	NULL	0	NULL	synaptotagmin			binds			C2B domain		PIP2					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1152_s_77	12738684	28 The C2B domain of synaptotagmin binds PIP2 preferentially to other phosphoinositides after exposure to Ca2+.	bind
30509	2	7510	7	NULL	NULL	0	NULL	Synaptotagmin	NULL		binds	NULL		C2B domain		phosphoinositides	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1152_s_77	12738684	28 The C2B domain of synaptotagmin binds PIP2 preferentially to other phosphoinositides after exposure to Ca2+.	bind
30510	3	7510	7	NULL	NULL	0	NULL	statement 1	NULL	binding of	is preferred than	NULL				statement 2	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1152_s_77	12738684	28 The C2B domain of synaptotagmin binds PIP2 preferentially to other phosphoinositides after exposure to Ca2+.	bind
30511	4	7510	7	NULL	NULL	0	NULL	statement 1	NULL		occurs after	NULL				Ca2+	NULL	exposure to			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1152_s_77	12738684	28 The C2B domain of synaptotagmin binds PIP2 preferentially to other phosphoinositides after exposure to Ca2+.	bind
30512	5	7510	7	NULL	NULL	0	NULL	statement 2	NULL		occurs after	NULL				Ca2+	NULL	exposure to			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1152_s_77	12738684	28 The C2B domain of synaptotagmin binds PIP2 preferentially to other phosphoinositides after exposure to Ca2+.	bind
31554	1	7511	5	13	NULL	NULL	NULL	cMyBP-C	GP		is homologus to			N-terminus		ELC-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_10_1290_s_170	16614305	28 The N-terminal homology of cMyBP-C with ELC-1 raises the possibility that the pro/ala-rich sequence of the C0C1 domain could, by interfering with these interactions between ELC-1 and the S1 heads, free some of the heads and increase their flexibility, thereby promoting the binding of S1 to actin.	bind
31555	2	7511	5	13	NULL	NULL	NULL	ELC-1	GP		interacts with								S1 heads		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_10_1290_s_170	16614305	28 The N-terminal homology of cMyBP-C with ELC-1 raises the possibility that the pro/ala-rich sequence of the C0C1 domain could, by interfering with these interactions between ELC-1 and the S1 heads, free some of the heads and increase their flexibility, thereby promoting the binding of S1 to actin.	bind
31556	3	7511	5	13	NULL	NULL	NULL				bind			S1		actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_10_1290_s_170	16614305	28 The N-terminal homology of cMyBP-C with ELC-1 raises the possibility that the pro/ala-rich sequence of the C0C1 domain could, by interfering with these interactions between ELC-1 and the S1 heads, free some of the heads and increase their flexibility, thereby promoting the binding of S1 to actin.	bind
31557	4	7511	5	13	NULL	NULL	NULL	cMyBP-C	GP		contains			C0C1 domain		cMyBP-C	GP		pro/ala-rich sequence		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_10_1290_s_170	16614305	28 The N-terminal homology of cMyBP-C with ELC-1 raises the possibility that the pro/ala-rich sequence of the C0C1 domain could, by interfering with these interactions between ELC-1 and the S1 heads, free some of the heads and increase their flexibility, thereby promoting the binding of S1 to actin.	bind
31558	5	7511	5	13	NULL	NULL	NULL	statement 4	Process		interfere with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_10_1290_s_170	16614305	28 The N-terminal homology of cMyBP-C with ELC-1 raises the possibility that the pro/ala-rich sequence of the C0C1 domain could, by interfering with these interactions between ELC-1 and the S1 heads, free some of the heads and increase their flexibility, thereby promoting the binding of S1 to actin.	bind
31559	6	7511	5	13	NULL	NULL	NULL	statement 5	Process		promote					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_10_1290_s_170	16614305	28 The N-terminal homology of cMyBP-C with ELC-1 raises the possibility that the pro/ala-rich sequence of the C0C1 domain could, by interfering with these interactions between ELC-1 and the S1 heads, free some of the heads and increase their flexibility, thereby promoting the binding of S1 to actin.	bind
54564	7	7511	5	13	NULL	NULL	NULL	statement 5	Process		free								S1 heads		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_10_1290_s_170	16614305	28 The N-terminal homology of cMyBP-C with ELC-1 raises the possibility that the pro/ala-rich sequence of the C0C1 domain could, by interfering with these interactions between ELC-1 and the S1 heads, free some of the heads and increase their flexibility, thereby promoting the binding of S1 to actin.	bind
54565	8	7511	5	13	NULL	NULL	NULL	statement 5	Process		increases							flexibility of	S1 heads		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_10_1290_s_170	16614305	28 The N-terminal homology of cMyBP-C with ELC-1 raises the possibility that the pro/ala-rich sequence of the C0C1 domain could, by interfering with these interactions between ELC-1 and the S1 heads, free some of the heads and increase their flexibility, thereby promoting the binding of S1 to actin.	bind
30513	1	7511	7	10	NULL	0	NULL	ELC-1			interacts with								S1 heads		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_10_1290_s_170	16614305	28 The N-terminal homology of cMyBP-C with ELC-1 raises the possibility that the pro/ala-rich sequence of the C0C1 domain could, by interfering with these interactions between ELC-1 and the S1 heads, free some of the heads and increase their flexibility, thereby promoting the binding of S1 to actin.	bind
30514	2	7511	7	NULL	NULL	0	NULL	cMyBP-C 	NULL		is homologous to	NULL		N-terminal 		ELC-1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_10_1290_s_170	16614305	28 The N-terminal homology of cMyBP-C with ELC-1 raises the possibility that the pro/ala-rich sequence of the C0C1 domain could, by interfering with these interactions between ELC-1 and the S1 heads, free some of the heads and increase their flexibility, thereby promoting the binding of S1 to actin.	bind
30515	3	7511	7	NULL	NULL	0	NULL	cMyBP-C	NULL		interfere with	NULL	may	pro/ala-rich sequence of the C0C1 domain		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_10_1290_s_170	16614305	28 The N-terminal homology of cMyBP-C with ELC-1 raises the possibility that the pro/ala-rich sequence of the C0C1 domain could, by interfering with these interactions between ELC-1 and the S1 heads, free some of the heads and increase their flexibility, thereby promoting the binding of S1 to actin.	bind
30516	4	7511	7	10	NULL	0	NULL	statement 3			free								S1 heads		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_10_1290_s_170	16614305	28 The N-terminal homology of cMyBP-C with ELC-1 raises the possibility that the pro/ala-rich sequence of the C0C1 domain could, by interfering with these interactions between ELC-1 and the S1 heads, free some of the heads and increase their flexibility, thereby promoting the binding of S1 to actin.	bind
30517	5	7511	7	10	NULL	0	NULL	statement 3			increase							flexibility of	S1 heads		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_10_1290_s_170	16614305	28 The N-terminal homology of cMyBP-C with ELC-1 raises the possibility that the pro/ala-rich sequence of the C0C1 domain could, by interfering with these interactions between ELC-1 and the S1 heads, free some of the heads and increase their flexibility, thereby promoting the binding of S1 to actin.	bind
30518	6	7511	7	NULL	NULL	0	NULL	S1	NULL		binds	NULL				actin	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_10_1290_s_170	16614305	28 The N-terminal homology of cMyBP-C with ELC-1 raises the possibility that the pro/ala-rich sequence of the C0C1 domain could, by interfering with these interactions between ELC-1 and the S1 heads, free some of the heads and increase their flexibility, thereby promoting the binding of S1 to actin.	bind
30519	7	7511	7	NULL	NULL	0	NULL	statement 5	NULL		promotes	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_10_1290_s_170	16614305	28 The N-terminal homology of cMyBP-C with ELC-1 raises the possibility that the pro/ala-rich sequence of the C0C1 domain could, by interfering with these interactions between ELC-1 and the S1 heads, free some of the heads and increase their flexibility, thereby promoting the binding of S1 to actin.	bind
28242	1	7512	5	13	NULL	NULL	NULL	acute phase SAA	GP	murine	bind					RAGE	GP	cell surface			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_2_561_s_257	11485914	28, 29 In addition, it was recently shown that murine acute phase SAA and murine AA fibril proteins bind to a cell surface receptor of advanced glycation end products (RAGE), which is a signal transduction receptor and does not lead to the internalization of SAA/AA fibril proteins.	bind
28243	2	7512	5	13	NULL	NULL	NULL	RAGE	GP		is					receptor of advanced glycation end products	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_2_561_s_257	11485914	28, 29 In addition, it was recently shown that murine acute phase SAA and murine AA fibril proteins bind to a cell surface receptor of advanced glycation end products (RAGE), which is a signal transduction receptor and does not lead to the internalization of SAA/AA fibril proteins.	bind
28244	3	7512	5	13	NULL	NULL	NULL	AA fibril proteins	GP	murine	bind					RAGE	GP	cell surface			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_2_561_s_257	11485914	28, 29 In addition, it was recently shown that murine acute phase SAA and murine AA fibril proteins bind to a cell surface receptor of advanced glycation end products (RAGE), which is a signal transduction receptor and does not lead to the internalization of SAA/AA fibril proteins.	bind
28245	4	7512	5	13	NULL	NULL	NULL	RAGE	GP		is a type of					signal transduction receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_2_561_s_257	11485914	28, 29 In addition, it was recently shown that murine acute phase SAA and murine AA fibril proteins bind to a cell surface receptor of advanced glycation end products (RAGE), which is a signal transduction receptor and does not lead to the internalization of SAA/AA fibril proteins.	bind
28246	5	7512	5	13	NULL	NULL	NULL	statement 1	Process		does not lead to					SAA/AA fibril proteins	GP	internalization of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_2_561_s_257	11485914	28, 29 In addition, it was recently shown that murine acute phase SAA and murine AA fibril proteins bind to a cell surface receptor of advanced glycation end products (RAGE), which is a signal transduction receptor and does not lead to the internalization of SAA/AA fibril proteins.	bind
28247	6	7512	5	13	NULL	NULL	NULL	statement 3	Process		does not lead to					SAA/AA fibril proteins	GP	internalization of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_2_561_s_257	11485914	28, 29 In addition, it was recently shown that murine acute phase SAA and murine AA fibril proteins bind to a cell surface receptor of advanced glycation end products (RAGE), which is a signal transduction receptor and does not lead to the internalization of SAA/AA fibril proteins.	bind
30520	1	7512	7	NULL	NULL	0	NULL	acute phase SAA proteins	NULL	murine 	bind	NULL				RAGE	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_2_561_s_257	11485914	28, 29 In addition, it was recently shown that murine acute phase SAA and murine AA fibril proteins bind to a cell surface receptor of advanced glycation end products (RAGE), which is a signal transduction receptor and does not lead to the internalization of SAA/AA fibril proteins.	bind
30521	2	7512	7	NULL	NULL	0	NULL	AA fibril proteins	NULL	murine	bind	NULL				RAGE	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_2_561_s_257	11485914	28, 29 In addition, it was recently shown that murine acute phase SAA and murine AA fibril proteins bind to a cell surface receptor of advanced glycation end products (RAGE), which is a signal transduction receptor and does not lead to the internalization of SAA/AA fibril proteins.	bind
30522	3	7512	7	NULL	NULL	0	NULL	RAGE	NULL		is	NULL				cell surface receptor of advanced glycation end products	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_2_561_s_257	11485914	28, 29 In addition, it was recently shown that murine acute phase SAA and murine AA fibril proteins bind to a cell surface receptor of advanced glycation end products (RAGE), which is a signal transduction receptor and does not lead to the internalization of SAA/AA fibril proteins.	bind
30523	4	7512	7	NULL	NULL	0	NULL	RAGE	NULL		is a type of	NULL				signal transduction receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_2_561_s_257	11485914	28, 29 In addition, it was recently shown that murine acute phase SAA and murine AA fibril proteins bind to a cell surface receptor of advanced glycation end products (RAGE), which is a signal transduction receptor and does not lead to the internalization of SAA/AA fibril proteins.	bind
30524	5	7512	7	NULL	NULL	0	NULL	statement 1	NULL		does not lead to	NULL				SAA/AA fibril proteins	NULL	internalization of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_2_561_s_257	11485914	28, 29 In addition, it was recently shown that murine acute phase SAA and murine AA fibril proteins bind to a cell surface receptor of advanced glycation end products (RAGE), which is a signal transduction receptor and does not lead to the internalization of SAA/AA fibril proteins.	bind
30525	6	7512	7	NULL	NULL	0	NULL	statement 2	NULL		does not lead to	NULL				SAA/AA fibril proteins	NULL	internalization of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_2_561_s_257	11485914	28, 29 In addition, it was recently shown that murine acute phase SAA and murine AA fibril proteins bind to a cell surface receptor of advanced glycation end products (RAGE), which is a signal transduction receptor and does not lead to the internalization of SAA/AA fibril proteins.	bind
31560	1	7513	5	13	NULL	NULL	NULL	PMEA	Chemical		is delivered to		selectively			macrophages	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_47_6_819_s_29	11389114	28, 29 In order to increase the selective delivery of PMEA to macrophages, a compound consisting of two molecules of PMEA bound together {di (P1,P2)[2-(adenin-9-yl)ethoxymethyl]phosphonate} (Bis-PMEA) was synthesized and encapsulated into autologous erythrocytes modified to increase their recognition and phagocytosis by human macrophages.	bind
30527	1	7513	7	10	NULL	0	NULL	PMEA			is delivered to		selectively			macrophages					NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_47_6_819_s_29	11389114	28, 29 In order to increase the selective delivery of PMEA to macrophages, a compound consisting of two molecules of PMEA bound together {di (P1,P2)[2-(adenin-9-yl)ethoxymethyl]phosphonate} (Bis-PMEA) was synthesized and encapsulated into autologous erythrocytes modified to increase their recognition and phagocytosis by human macrophages.	bind
28248	1	7514	5	13	NULL	NULL	NULL	gp91 phox	GP		bind					p47 phox	GP				NULL	in human neutrophils	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_5_776_s_32	12637340	28,29  In human neutrophils, small peptide sequences of gp91 phox, which are involved in the binding of gp91 phox to p47 phox, inhibit O2.	bind
28249	2	7514	5	13	NULL	NULL	NULL	gp91 phox	GP	small peptide sequences of	is involved in					statement 1	Process				NULL	in human neutrophils	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_5_776_s_32	12637340	28,29  In human neutrophils, small peptide sequences of gp91 phox, which are involved in the binding of gp91 phox to p47 phox, inhibit O2.	bind
28250	3	7514	5	13	NULL	NULL	NULL	gp91 phox	GP	small peptide sequences of	inhibit					O2	Chemical				NULL	in human neutrophils	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_5_776_s_32	12637340	28,29  In human neutrophils, small peptide sequences of gp91 phox, which are involved in the binding of gp91 phox to p47 phox, inhibit O2.	bind
30542	1	7514	7	NULL	NULL	0	NULL	gp91 phox	NULL		bind	NULL				p47phox	NULL				NULL	human neutrophils	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_5_776_s_32	12637340	28,29  In human neutrophils, small peptide sequences of gp91 phox, which are involved in the binding of gp91 phox to p47 phox, inhibit O2.	bind
30543	2	7514	7	10	NULL	0	NULL	gp91 phox		 small peptide sequences of	is involved in					statement 1					NULL	human neutrophils	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_5_776_s_32	12637340	28,29  In human neutrophils, small peptide sequences of gp91 phox, which are involved in the binding of gp91 phox to p47 phox, inhibit O2.	bind
30544	3	7514	7	10	NULL	0	NULL	gp91 phox	NULL	small peptide sequences of	inhibit	NULL				O2	NULL				NULL	human neutrophils	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_5_776_s_32	12637340	28,29  In human neutrophils, small peptide sequences of gp91 phox, which are involved in the binding of gp91 phox to p47 phox, inhibit O2.	bind
28251	1	7515	5	13	NULL	NULL	NULL	Nebulin	GP	sequence of	is similar to					nebulette	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_66	14976140	28,33  Nebulin and nebulette share sequence similarities and contain 35 residue repeats (nebulin repeats), a linker domain, and a C-terminal Src homology 3 (SH3) domain that also binds to alpha-actinin.	bind
46654	2	7515	5	13	NULL	NULL	NULL	Nebulin	GP		contains								nebulin repeats		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_66	14976140	28,33  Nebulin and nebulette share sequence similarities and contain 35 residue repeats (nebulin repeats), a linker domain, and a C-terminal Src homology 3 (SH3) domain that also binds to alpha-actinin.	bind
46674	3	7515	5	13	NULL	NULL	NULL	Nebulin	GP		contains								linker domain		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_66	14976140	28,33  Nebulin and nebulette share sequence similarities and contain 35 residue repeats (nebulin repeats), a linker domain, and a C-terminal Src homology 3 (SH3) domain that also binds to alpha-actinin.	bind
46675	4	7515	5	13	NULL	NULL	NULL	Nebulin	GP		contains								C-terminal SH3		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_66	14976140	28,33  Nebulin and nebulette share sequence similarities and contain 35 residue repeats (nebulin repeats), a linker domain, and a C-terminal Src homology 3 (SH3) domain that also binds to alpha-actinin.	bind
46676	5	7515	5	13	NULL	NULL	NULL	nebulin repeats	GP		contains								35 residue repeats		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_66	14976140	28,33  Nebulin and nebulette share sequence similarities and contain 35 residue repeats (nebulin repeats), a linker domain, and a C-terminal Src homology 3 (SH3) domain that also binds to alpha-actinin.	bind
46677	6	7515	5	13	NULL	NULL	NULL	nebulette	GP		contains								nebulin repeats		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_66	14976140	28,33  Nebulin and nebulette share sequence similarities and contain 35 residue repeats (nebulin repeats), a linker domain, and a C-terminal Src homology 3 (SH3) domain that also binds to alpha-actinin.	bind
46678	7	7515	5	13	NULL	NULL	NULL	nebulette	GP		contains								linker domain		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_66	14976140	28,33  Nebulin and nebulette share sequence similarities and contain 35 residue repeats (nebulin repeats), a linker domain, and a C-terminal Src homology 3 (SH3) domain that also binds to alpha-actinin.	bind
46679	8	7515	5	13	NULL	NULL	NULL	nebulette	GP		contains								C-terminal SH3		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_66	14976140	28,33  Nebulin and nebulette share sequence similarities and contain 35 residue repeats (nebulin repeats), a linker domain, and a C-terminal Src homology 3 (SH3) domain that also binds to alpha-actinin.	bind
46680	9	7515	5	13	NULL	NULL	NULL	nebulette	GP		bind			\tC-terminal SH3 domain		alpha-actinin	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_66	14976140	28,33  Nebulin and nebulette share sequence similarities and contain 35 residue repeats (nebulin repeats), a linker domain, and a C-terminal Src homology 3 (SH3) domain that also binds to alpha-actinin.	bind
46681	10	7515	5	13	NULL	NULL	NULL	Nebulin	GP		bind			\tC-terminal SH3 domain		alpha-actinin	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_66	14976140	28,33  Nebulin and nebulette share sequence similarities and contain 35 residue repeats (nebulin repeats), a linker domain, and a C-terminal Src homology 3 (SH3) domain that also binds to alpha-actinin.	bind
30545	1	7515	7	NULL	NULL	0	NULL	Nebulin 	NULL	sequence of	is similar to	NULL				nebulette	NULL	sequence of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_66	14976140	28,33  Nebulin and nebulette share sequence similarities and contain 35 residue repeats (nebulin repeats), a linker domain, and a C-terminal Src homology 3 (SH3) domain that also binds to alpha-actinin.	bind
30546	2	7515	7	NULL	NULL	0	NULL	Nebulin	NULL		contains	NULL					NULL		nebulin repeats		NULL		0	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_66	14976140	28,33  Nebulin and nebulette share sequence similarities and contain 35 residue repeats (nebulin repeats), a linker domain, and a C-terminal Src homology 3 (SH3) domain that also binds to alpha-actinin.	bind
30547	3	7515	7	NULL	NULL	0	NULL	Nebulin	NULL		contains	NULL					NULL		linker domain		NULL		0	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_66	14976140	28,33  Nebulin and nebulette share sequence similarities and contain 35 residue repeats (nebulin repeats), a linker domain, and a C-terminal Src homology 3 (SH3) domain that also binds to alpha-actinin.	bind
30548	4	7515	7	NULL	NULL	0	NULL	Nebulin			contains								 C-terminal SH3 domain		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_66	14976140	28,33  Nebulin and nebulette share sequence similarities and contain 35 residue repeats (nebulin repeats), a linker domain, and a C-terminal Src homology 3 (SH3) domain that also binds to alpha-actinin.	bind
30549	5	7515	7	NULL	NULL	0	NULL	Nebulin			bind			C-terminal SH3 domain		alpha-actinin					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_66	14976140	28,33  Nebulin and nebulette share sequence similarities and contain 35 residue repeats (nebulin repeats), a linker domain, and a C-terminal Src homology 3 (SH3) domain that also binds to alpha-actinin.	bind
30553	6	7515	7	NULL	NULL	0	NULL	nebulin repeats	NULL		contains	NULL					NULL		35 residue repeats 		NULL		0	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_66	14976140	28,33  Nebulin and nebulette share sequence similarities and contain 35 residue repeats (nebulin repeats), a linker domain, and a C-terminal Src homology 3 (SH3) domain that also binds to alpha-actinin.	bind
30554	7	7515	7	NULL	NULL	0	NULL	SH3	NULL		is	NULL				 Src homology 3 	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_66	14976140	28,33  Nebulin and nebulette share sequence similarities and contain 35 residue repeats (nebulin repeats), a linker domain, and a C-terminal Src homology 3 (SH3) domain that also binds to alpha-actinin.	bind
54818	8	7515	7	NULL	NULL	0	NULL	nebulette			contains					nebulin repeats					NULL		0	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_66	14976140	28,33  Nebulin and nebulette share sequence similarities and contain 35 residue repeats (nebulin repeats), a linker domain, and a C-terminal Src homology 3 (SH3) domain that also binds to alpha-actinin.	bind
54819	9	7515	7	NULL	NULL	0	NULL	nebulette			contains					 linker domain					NULL		0	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_66	14976140	28,33  Nebulin and nebulette share sequence similarities and contain 35 residue repeats (nebulin repeats), a linker domain, and a C-terminal Src homology 3 (SH3) domain that also binds to alpha-actinin.	bind
54820	10	7515	7	NULL	NULL	0	NULL	nebulette			contains								C-terminal SH3 domain		NULL		0	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_66	14976140	28,33  Nebulin and nebulette share sequence similarities and contain 35 residue repeats (nebulin repeats), a linker domain, and a C-terminal Src homology 3 (SH3) domain that also binds to alpha-actinin.	bind
54821	11	7515	7	NULL	NULL	0	NULL	nebulette			bind			C-terminal SH3 domain		alpha-actinin					NULL		0	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_66	14976140	28,33  Nebulin and nebulette share sequence similarities and contain 35 residue repeats (nebulin repeats), a linker domain, and a C-terminal Src homology 3 (SH3) domain that also binds to alpha-actinin.	bind
28252	1	7516	5	13	NULL	NULL	NULL	LPS	Chemical		bind					TLR4	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_24_21129_s_204	11274165	28C5 blocks  LPS  binding to TLR4 and MD-2.	bind
28253	2	7516	5	13	NULL	NULL	NULL	28C5	Chemical		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_24_21129_s_204	11274165	28C5 blocks  LPS  binding to TLR4 and MD-2.	bind
28254	3	7516	5	13	NULL	NULL	NULL	LPS	Chemical		bind					MD-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_24_21129_s_204	11274165	28C5 blocks  LPS  binding to TLR4 and MD-2.	bind
28255	4	7516	5	13	NULL	NULL	NULL	28C5	Chemical		blocks					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_24_21129_s_204	11274165	28C5 blocks  LPS  binding to TLR4 and MD-2.	bind
28258	3	7516	5	13	NULL	NULL	NULL	MY-4	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_24_21129_s_204	11274165	28C5 blocks  LPS  binding to TLR4 and MD-2.	bind
30570	1	7516	7	NULL	NULL	0	NULL	LPS	NULL		binds to	NULL				TLR4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_24_21129_s_204	11274165	28C5 blocks  LPS  binding to TLR4 and MD-2.	bind
30571	2	7516	7	NULL	NULL	0	NULL	LPS	NULL		binds to	NULL				MD-2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_24_21129_s_204	11274165	28C5 blocks  LPS  binding to TLR4 and MD-2.	bind
30573	3	7516	7	NULL	NULL	0	NULL	28C5	NULL		blocks	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_24_21129_s_204	11274165	28C5 blocks  LPS  binding to TLR4 and MD-2.	bind
30574	4	7516	7	NULL	NULL	0	NULL	28C5	NULL		blocks	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_24_21129_s_204	11274165	28C5 blocks  LPS  binding to TLR4 and MD-2.	bind
28256	1	7517	5	13	NULL	NULL	NULL	CD14	GP		bind					LPS	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3144_s_110	10652298	28C5, MY-4, and 60bca have been shown to inhibit CD14 binding to LPS ( 10,  26).	bind
28257	2	7517	5	13	NULL	NULL	NULL	28C5	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3144_s_110	10652298	28C5, MY-4, and 60bca have been shown to inhibit CD14 binding to LPS ( 10,  26).	bind
28259	4	7517	5	13	NULL	NULL	NULL	60bca	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3144_s_110	10652298	28C5, MY-4, and 60bca have been shown to inhibit CD14 binding to LPS ( 10,  26).	bind
30580	1	7517	7	NULL	NULL	0	NULL	CD14	NULL		binds to	NULL				LPS	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_5_3144_s_110	10652298	28C5, MY-4, and 60bca have been shown to inhibit CD14 binding to LPS ( 10,  26).	bind
30581	2	7517	7	NULL	NULL	0	NULL	28C5	NULL		inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_5_3144_s_110	10652298	28C5, MY-4, and 60bca have been shown to inhibit CD14 binding to LPS ( 10,  26).	bind
30582	3	7517	7	NULL	NULL	0	NULL	MY-4	NULL		inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_5_3144_s_110	10652298	28C5, MY-4, and 60bca have been shown to inhibit CD14 binding to LPS ( 10,  26).	bind
30583	4	7517	7	NULL	NULL	0	NULL	60bca	NULL		inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_5_3144_s_110	10652298	28C5, MY-4, and 60bca have been shown to inhibit CD14 binding to LPS ( 10,  26).	bind
28260	1	7518	5	13	NULL	NULL	NULL	spermine molecule	Chemical		bind					Z-DNA	NucleicAcid			minor groove	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_419_s_441	11788703	29       Bancroft,D., Williams,L.D., Rich,A. and Egli,M. (1994) The  low-temperature crystal structure of the pure-spermine form of Z-DNA reveals binding of a spermine molecule in the minor groove.	bind
28261	2	7518	5	13	NULL	NULL	NULL	statement 1	Process		occurs in					low-temperature					NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_419_s_441	11788703	29       Bancroft,D., Williams,L.D., Rich,A. and Egli,M. (1994) The  low-temperature crystal structure of the pure-spermine form of Z-DNA reveals binding of a spermine molecule in the minor groove.	bind
30585	1	7518	7	NULL	NULL	0	NULL	 spermine molecule	NULL	pure	binds to	NULL				Z-DNA	NULL			minor groove	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_419_s_441	11788703	29       Bancroft,D., Williams,L.D., Rich,A. and Egli,M. (1994) The  low-temperature crystal structure of the pure-spermine form of Z-DNA reveals binding of a spermine molecule in the minor groove.	bind
28398	1	7519	5	13	NULL	NULL	NULL	Sos1	GP	human	is a type of					guanine nucleotide exchange factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_6_1300_s_345	11238996	29       Chardin,P., Camonis,J.H., Gale,N.W., van Aelst,L., Schlessinger,J., Wigler,M.H. and Bar-Sagi,D. (1993) Human Sos1: a guanine nucleotide exchange factor for Ras that binds to Grb2.	bind
30438	2	7519	5	13	NULL	NULL	NULL	Sos1	GP	human	bind					Grb2	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_6_1300_s_345	11238996	29       Chardin,P., Camonis,J.H., Gale,N.W., van Aelst,L., Schlessinger,J., Wigler,M.H. and Bar-Sagi,D. (1993) Human Sos1: a guanine nucleotide exchange factor for Ras that binds to Grb2.	bind
30586	1	7519	7	NULL	NULL	0	NULL	Sos1	NULL	human	binds to	NULL				Grb2	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_6_1300_s_345	11238996	29       Chardin,P., Camonis,J.H., Gale,N.W., van Aelst,L., Schlessinger,J., Wigler,M.H. and Bar-Sagi,D. (1993) Human Sos1: a guanine nucleotide exchange factor for Ras that binds to Grb2.	bind
30587	2	7519	7	NULL	NULL	0	NULL	Sos1	NULL	human	is a type of	NULL				guanine nucleotide exchange factor for Ras	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_6_1300_s_345	11238996	29       Chardin,P., Camonis,J.H., Gale,N.W., van Aelst,L., Schlessinger,J., Wigler,M.H. and Bar-Sagi,D. (1993) Human Sos1: a guanine nucleotide exchange factor for Ras that binds to Grb2.	bind
28400	1	7520	5	13	NULL	NULL	NULL	WT1	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_24_4865_s_326	11121477	29       Hamilton,T.B., Borel,F. and Romaniuk,P.J. (1998) Comparison of the DNA binding characteristics of the related zinc finger proteins WT1 and EGR1.	bind
28401	2	7520	5	13	NULL	NULL	NULL	EGR1	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_24_4865_s_326	11121477	29       Hamilton,T.B., Borel,F. and Romaniuk,P.J. (1998) Comparison of the DNA binding characteristics of the related zinc finger proteins WT1 and EGR1.	bind
28402	3	7520	5	13	NULL	NULL	NULL	EGR1	GP		is a type of					zinc finger proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_24_4865_s_326	11121477	29       Hamilton,T.B., Borel,F. and Romaniuk,P.J. (1998) Comparison of the DNA binding characteristics of the related zinc finger proteins WT1 and EGR1.	bind
28403	4	7520	5	13	NULL	NULL	NULL	WT1	GP		is a type of					zinc finger proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_24_4865_s_326	11121477	29       Hamilton,T.B., Borel,F. and Romaniuk,P.J. (1998) Comparison of the DNA binding characteristics of the related zinc finger proteins WT1 and EGR1.	bind
30592	1	7520	7	NULL	NULL	0	NULL	WT1	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_24_4865_s_326	11121477	29       Hamilton,T.B., Borel,F. and Romaniuk,P.J. (1998) Comparison of the DNA binding characteristics of the related zinc finger proteins WT1 and EGR1.	bind
30593	2	7520	7	NULL	NULL	0	NULL	EGR1	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_24_4865_s_326	11121477	29       Hamilton,T.B., Borel,F. and Romaniuk,P.J. (1998) Comparison of the DNA binding characteristics of the related zinc finger proteins WT1 and EGR1.	bind
30594	3	7520	7	NULL	NULL	0	NULL	WT1	NULL		is a type of	NULL				zinc finger protein	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_24_4865_s_326	11121477	29       Hamilton,T.B., Borel,F. and Romaniuk,P.J. (1998) Comparison of the DNA binding characteristics of the related zinc finger proteins WT1 and EGR1.	bind
30595	4	7520	7	NULL	NULL	0	NULL	EGR1	NULL		is a type of	NULL				zinc finger protein	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_24_4865_s_326	11121477	29       Hamilton,T.B., Borel,F. and Romaniuk,P.J. (1998) Comparison of the DNA binding characteristics of the related zinc finger proteins WT1 and EGR1.	bind
28404	1	7521	5	13	NULL	NULL	NULL	Pur factor	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_17_3197_s_348	10954586	29       Herault,Y., Chatelain,G., Brum,G. and Michel,D. (1995) RNA-dependent DNA binding activity of the Pur factor, potentially involved in DNA replication and gene transcription.	bind
28407	2	7521	5	13	NULL	NULL	NULL	statement 1	Process		is dependent on					RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_17_3197_s_348	10954586	29       Herault,Y., Chatelain,G., Brum,G. and Michel,D. (1995) RNA-dependent DNA binding activity of the Pur factor, potentially involved in DNA replication and gene transcription.	bind
28410	3	7521	5	13	NULL	NULL	NULL	statement 1	Process		is involved in		potentially			DNA	NucleicAcid	replication of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_17_3197_s_348	10954586	29       Herault,Y., Chatelain,G., Brum,G. and Michel,D. (1995) RNA-dependent DNA binding activity of the Pur factor, potentially involved in DNA replication and gene transcription.	bind
54531	4	7521	5	13	NULL	NULL	NULL	statement 1	Process		is involved in		potentially			gene	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_17_3197_s_348	10954586	29       Herault,Y., Chatelain,G., Brum,G. and Michel,D. (1995) RNA-dependent DNA binding activity of the Pur factor, potentially involved in DNA replication and gene transcription.	bind
30597	1	7521	7	NULL	NULL	0	NULL	Pur factor	NULL		binds	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_17_3197_s_348	10954586	29       Herault,Y., Chatelain,G., Brum,G. and Michel,D. (1995) RNA-dependent DNA binding activity of the Pur factor, potentially involved in DNA replication and gene transcription.	bind
30598	2	7521	7	NULL	NULL	0	NULL	statement 1	NULL		depends on	NULL				RNA	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_17_3197_s_348	10954586	29       Herault,Y., Chatelain,G., Brum,G. and Michel,D. (1995) RNA-dependent DNA binding activity of the Pur factor, potentially involved in DNA replication and gene transcription.	bind
30599	3	7521	7	10	NULL	0	NULL	statement 1			is involved in		potentially			DNA		replication of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_17_3197_s_348	10954586	29       Herault,Y., Chatelain,G., Brum,G. and Michel,D. (1995) RNA-dependent DNA binding activity of the Pur factor, potentially involved in DNA replication and gene transcription.	bind
30600	4	7521	7	10	NULL	0	NULL	statement 1			is involved in		potentially			gene		transcription of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_17_3197_s_348	10954586	29       Herault,Y., Chatelain,G., Brum,G. and Michel,D. (1995) RNA-dependent DNA binding activity of the Pur factor, potentially involved in DNA replication and gene transcription.	bind
28413	1	7522	5	13	NULL	NULL	NULL	nuclear proteins	GP		bind							cauliflower mosaic virus		35S truncated promoter	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_3_775_s_283	11809891	29       Prat,S., Willmitzer,L. and Sanchez-Serrano,J.J. (1989) Nuclear proteins binding to a cauliflower mosaic virus 35S truncated promoter.	bind
30632	1	7522	7	NULL	NULL	0	NULL	Nuclear proteins	NULL		binds to	NULL					NULL	cauliflower mosaic virus		35S truncated promoter	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_3_775_s_283	11809891	29       Prat,S., Willmitzer,L. and Sanchez-Serrano,J.J. (1989) Nuclear proteins binding to a cauliflower mosaic virus 35S truncated promoter.	bind
28414	1	7523	5	13	NULL	NULL	NULL	NGFI-A	GP		bind		specifically			DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_4920_s_330	11812820	29       Swirnoff,A.H. and Milbrandt,J. (1995) DNA-binding specificity of NGFI-A and related zinc finger transcription factors.	bind
30633	1	7523	7	10	NULL	0	NULL	NGFI-A 			bind		specifically			DNA					NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_4920_s_330	11812820	29       Swirnoff,A.H. and Milbrandt,J. (1995) DNA-binding specificity of NGFI-A and related zinc finger transcription factors.	bind
28415	1	7524	5	13	NULL	NULL	NULL	TFIIIA	GP		bind					class III genes	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_767_s_355	11160900	29       Van Dyke,M.W. and Roeder,R.G. (1987) Novobiocin interferes with the binding of transcription factors TFIIIA and TFIIIC to the promoters of class III genes.	bind
28416	2	7524	5	13	NULL	NULL	NULL	TFIIIC	GP		bind					class III genes	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_767_s_355	11160900	29       Van Dyke,M.W. and Roeder,R.G. (1987) Novobiocin interferes with the binding of transcription factors TFIIIA and TFIIIC to the promoters of class III genes.	bind
28417	3	7524	5	13	NULL	NULL	NULL	TFIIIA	GP		is a type of					transcription facor	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_767_s_355	11160900	29       Van Dyke,M.W. and Roeder,R.G. (1987) Novobiocin interferes with the binding of transcription factors TFIIIA and TFIIIC to the promoters of class III genes.	bind
28418	4	7524	5	13	NULL	NULL	NULL	TFIIIC	GP		is a type of					transcription facor	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_767_s_355	11160900	29       Van Dyke,M.W. and Roeder,R.G. (1987) Novobiocin interferes with the binding of transcription factors TFIIIA and TFIIIC to the promoters of class III genes.	bind
28419	5	7524	5	13	NULL	NULL	NULL	novobiocin	Chemical		interferes with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_767_s_355	11160900	29       Van Dyke,M.W. and Roeder,R.G. (1987) Novobiocin interferes with the binding of transcription factors TFIIIA and TFIIIC to the promoters of class III genes.	bind
28420	6	7524	5	13	NULL	NULL	NULL	novobiocin	Chemical		interferes with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_767_s_355	11160900	29       Van Dyke,M.W. and Roeder,R.G. (1987) Novobiocin interferes with the binding of transcription factors TFIIIA and TFIIIC to the promoters of class III genes.	bind
30635	1	7524	7	NULL	NULL	0	NULL	TFIIIA	NULL		binds	NULL				class III genes	NULL			promoters of	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_767_s_355	11160900	29       Van Dyke,M.W. and Roeder,R.G. (1987) Novobiocin interferes with the binding of transcription factors TFIIIA and TFIIIC to the promoters of class III genes.	bind
30636	2	7524	7	NULL	NULL	0	NULL	TFIIIC	NULL		binds	NULL				class III genes	NULL			promoters of	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_767_s_355	11160900	29       Van Dyke,M.W. and Roeder,R.G. (1987) Novobiocin interferes with the binding of transcription factors TFIIIA and TFIIIC to the promoters of class III genes.	bind
30637	3	7524	7	NULL	NULL	0	NULL	Novobiocin	NULL		interferes with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_767_s_355	11160900	29       Van Dyke,M.W. and Roeder,R.G. (1987) Novobiocin interferes with the binding of transcription factors TFIIIA and TFIIIC to the promoters of class III genes.	bind
30638	4	7524	7	NULL	NULL	0	NULL	Novobiocin	NULL		interferes with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_767_s_355	11160900	29       Van Dyke,M.W. and Roeder,R.G. (1987) Novobiocin interferes with the binding of transcription factors TFIIIA and TFIIIC to the promoters of class III genes.	bind
30639	5	7524	7	NULL	NULL	0	NULL	TFIIIA	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_767_s_355	11160900	29       Van Dyke,M.W. and Roeder,R.G. (1987) Novobiocin interferes with the binding of transcription factors TFIIIA and TFIIIC to the promoters of class III genes.	bind
30640	6	7524	7	NULL	NULL	0	NULL	TFIIIC	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_767_s_355	11160900	29       Van Dyke,M.W. and Roeder,R.G. (1987) Novobiocin interferes with the binding of transcription factors TFIIIA and TFIIIC to the promoters of class III genes.	bind
28422	1	7525	5	13	NULL	NULL	NULL	thrombin	GP		interacts with					TM	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_3_520_s_204	9102171	29  Alternatively, the anti-TM antibody may specifically alter the cofactor protein C function of TM by blocking the interaction between thrombin and TM, since the primary thrombin binding site of TM is thought to be composed of the fifth and sixth epidermal growth factor homology regions.	bind
28424	2	7525	5	13	NULL	NULL	NULL	TM	GP		contains					cofactor protein C function	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_3_520_s_204	9102171	29  Alternatively, the anti-TM antibody may specifically alter the cofactor protein C function of TM by blocking the interaction between thrombin and TM, since the primary thrombin binding site of TM is thought to be composed of the fifth and sixth epidermal growth factor homology regions.	bind
28425	3	7525	5	13	NULL	NULL	NULL	anti-TM antibody	GP		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_3_520_s_204	9102171	29  Alternatively, the anti-TM antibody may specifically alter the cofactor protein C function of TM by blocking the interaction between thrombin and TM, since the primary thrombin binding site of TM is thought to be composed of the fifth and sixth epidermal growth factor homology regions.	bind
28428	4	7525	5	13	NULL	NULL	NULL	statement 3	Process		alters		may;;specifically			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_3_520_s_204	9102171	29  Alternatively, the anti-TM antibody may specifically alter the cofactor protein C function of TM by blocking the interaction between thrombin and TM, since the primary thrombin binding site of TM is thought to be composed of the fifth and sixth epidermal growth factor homology regions.	bind
28429	5	7525	5	13	NULL	NULL	NULL	TM	GP	primary	is composed of			thrombin binding site					fifth epidermal growth factor homology region		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_3_520_s_204	9102171	29  Alternatively, the anti-TM antibody may specifically alter the cofactor protein C function of TM by blocking the interaction between thrombin and TM, since the primary thrombin binding site of TM is thought to be composed of the fifth and sixth epidermal growth factor homology regions.	bind
46655	6	7525	5	13	NULL	NULL	NULL	TM	GP	primary	is composed of			thrombin binding site					sixth epidermal growth factor homology regions		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_3_520_s_204	9102171	29  Alternatively, the anti-TM antibody may specifically alter the cofactor protein C function of TM by blocking the interaction between thrombin and TM, since the primary thrombin binding site of TM is thought to be composed of the fifth and sixth epidermal growth factor homology regions.	bind
30644	1	7525	7	10	NULL	0	NULL	 anti-TM antibody			alter		specifically			statement 6					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_3_520_s_204	9102171	29  Alternatively, the anti-TM antibody may specifically alter the cofactor protein C function of TM by blocking the interaction between thrombin and TM, since the primary thrombin binding site of TM is thought to be composed of the fifth and sixth epidermal growth factor homology regions.	bind
30647	2	7525	7	NULL	NULL	0	NULL	thrombin	NULL		interacts with	NULL				TM	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_3_520_s_204	9102171	29  Alternatively, the anti-TM antibody may specifically alter the cofactor protein C function of TM by blocking the interaction between thrombin and TM, since the primary thrombin binding site of TM is thought to be composed of the fifth and sixth epidermal growth factor homology regions.	bind
30649	3	7525	7	NULL	NULL	0	NULL	statement 1	NULL		occurs by blocking	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_3_520_s_204	9102171	29  Alternatively, the anti-TM antibody may specifically alter the cofactor protein C function of TM by blocking the interaction between thrombin and TM, since the primary thrombin binding site of TM is thought to be composed of the fifth and sixth epidermal growth factor homology regions.	bind
30650	4	7525	7	10	NULL	0	NULL	TM	NULL	primary	is composed of	NULL		thrombin binding site			NULL		fifth epidermal growth factor homology region		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_3_520_s_204	9102171	29  Alternatively, the anti-TM antibody may specifically alter the cofactor protein C function of TM by blocking the interaction between thrombin and TM, since the primary thrombin binding site of TM is thought to be composed of the fifth and sixth epidermal growth factor homology regions.	bind
30652	5	7525	7	10	NULL	0	NULL	TM	NULL	primary	is composed of	NULL		thrombin binding site			NULL		 sixth epidermal growth factor homology region		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_3_520_s_204	9102171	29  Alternatively, the anti-TM antibody may specifically alter the cofactor protein C function of TM by blocking the interaction between thrombin and TM, since the primary thrombin binding site of TM is thought to be composed of the fifth and sixth epidermal growth factor homology regions.	bind
54532	6	7525	7	10	NULL	0	NULL	TM			contains					cofactor protein C function					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_3_520_s_204	9102171	29  Alternatively, the anti-TM antibody may specifically alter the cofactor protein C function of TM by blocking the interaction between thrombin and TM, since the primary thrombin binding site of TM is thought to be composed of the fifth and sixth epidermal growth factor homology regions.	bind
28431	1	7526	5	13	NULL	NULL	NULL	AT1 receptor	GP		is a type of					G protein - coupled receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_6_1053_s_168	7586216	29  Although the AT1 receptor is a typical G protein - coupled receptor in that it lacks tyrosine kinase activity, many proteins are rapidly tyrosine-phosphorylated when Ang II binds to the AT1 receptor.	bind
28433	2	7526	5	13	NULL	NULL	NULL	AT1 receptor	GP		lacks					tyrosine kinase activity	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_6_1053_s_168	7586216	29  Although the AT1 receptor is a typical G protein - coupled receptor in that it lacks tyrosine kinase activity, many proteins are rapidly tyrosine-phosphorylated when Ang II binds to the AT1 receptor.	bind
28435	3	7526	5	13	NULL	NULL	NULL	Ang II	GP		bind					AT1 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_6_1053_s_168	7586216	29  Although the AT1 receptor is a typical G protein - coupled receptor in that it lacks tyrosine kinase activity, many proteins are rapidly tyrosine-phosphorylated when Ang II binds to the AT1 receptor.	bind
30666	1	7526	7	NULL	NULL	0	NULL	Ang II	NULL		binds to	NULL				AT1 receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_77_6_1053_s_168	7586216	29  Although the AT1 receptor is a typical G protein - coupled receptor in that it lacks tyrosine kinase activity, many proteins are rapidly tyrosine-phosphorylated when Ang II binds to the AT1 receptor.	bind
30668	3	7526	7	NULL	NULL	0	NULL	 AT1 receptor	NULL		is a type of	NULL				G protein - coupled receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_77_6_1053_s_168	7586216	29  Although the AT1 receptor is a typical G protein - coupled receptor in that it lacks tyrosine kinase activity, many proteins are rapidly tyrosine-phosphorylated when Ang II binds to the AT1 receptor.	bind
30669	4	7526	7	NULL	NULL	0	NULL	AT1 receptor	NULL		lacks	NULL				tyrosine kinase activity	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_77_6_1053_s_168	7586216	29  Although the AT1 receptor is a typical G protein - coupled receptor in that it lacks tyrosine kinase activity, many proteins are rapidly tyrosine-phosphorylated when Ang II binds to the AT1 receptor.	bind
28444	1	7527	5	13	NULL	NULL	NULL	Plg	GP		bind					Plg receptors	GP	surface			NULL	on endothelial cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_3_433_s_149	11231925	29  Lp(a) also interferes with Plg binding to the surface Plg receptors on endothelial cells.	bind
28445	2	7527	5	13	NULL	NULL	NULL	Lp(a)	GP		interferes with					statement 1	Process				NULL	endothelial cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_3_433_s_149	11231925	29  Lp(a) also interferes with Plg binding to the surface Plg receptors on endothelial cells.	bind
30670	1	7527	7	10	NULL	0	NULL	Plg			binds					Plg receptors		surface			NULL	endothelial cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_3_433_s_149	11231925	29  Lp(a) also interferes with Plg binding to the surface Plg receptors on endothelial cells.	bind
30671	2	7527	7	10	NULL	0	NULL	 Lp(a)			interferes with					statement 1					NULL	endothelial cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_3_433_s_149	11231925	29  Lp(a) also interferes with Plg binding to the surface Plg receptors on endothelial cells.	bind
28447	1	7528	5	13	NULL	NULL	NULL	mAb C-7	GP		bind					apoB/E receptor	GP				NULL	in human cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_149_s_101	9012650	29  mAb C-7, which binds to the apoB/E receptor in human cells, was used for binding competition studies.	bind
30672	1	7528	7	10	NULL	0	NULL	 mAb C-7	NULL		binds to	NULL				apoB/E receptor	NULL				NULL	human cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_149_s_101	9012650	29  mAb C-7, which binds to the apoB/E receptor in human cells, was used for binding competition studies.	bind
28450	1	7530	5	13	NULL	NULL	NULL	fibrinogen	GP		bind					platelet GPIIb/IIIa receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2535_s_170	10521384	29  XV459 has been shown to be a competitive inhibitor with high affinity for inhibiting fibrinogen binding to platelet GPIIb/IIIa receptors.	bind
28451	2	7530	5	13	NULL	NULL	NULL	XV459	Chemical		is a type of					competitive inhibitor	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2535_s_170	10521384	29  XV459 has been shown to be a competitive inhibitor with high affinity for inhibiting fibrinogen binding to platelet GPIIb/IIIa receptors.	bind
28453	3	7530	5	13	NULL	NULL	NULL	XV459	Chemical		inhibit		high affinity			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2535_s_170	10521384	29  XV459 has been shown to be a competitive inhibitor with high affinity for inhibiting fibrinogen binding to platelet GPIIb/IIIa receptors.	bind
30673	1	7530	7	NULL	NULL	0	NULL	fibrinogen	NULL		binds to	NULL				platelet GPIIb/IIIa receptors	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2535_s_170	10521384	29  XV459 has been shown to be a competitive inhibitor with high affinity for inhibiting fibrinogen binding to platelet GPIIb/IIIa receptors.	bind
30674	2	7530	7	10	NULL	0	NULL	XV459	NULL		inhibits	NULL	high affinity			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2535_s_170	10521384	29  XV459 has been shown to be a competitive inhibitor with high affinity for inhibiting fibrinogen binding to platelet GPIIb/IIIa receptors.	bind
54533	3	7530	7	10	NULL	0	NULL	XV459			is a type of					competitive inhibitor					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2535_s_170	10521384	29  XV459 has been shown to be a competitive inhibitor with high affinity for inhibiting fibrinogen binding to platelet GPIIb/IIIa receptors.	bind
28455	1	7531	5	13	NULL	NULL	NULL	ECSODR213G	GP		bind					collagen type I	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_7_1047_s_181	16087794	29 Despite the difference in the degree of binding observed previously 29 and in the present study, which may have resulted from different methods of detection, both studies indicate that ECSODR213G indeed binds to collagen type I.	bind
30915	1	7531	7	NULL	NULL	0	NULL	ECSODR213G	NULL		binds to	NULL				collagen type I	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_112_7_1047_s_181	16087794	29 Despite the difference in the degree of binding observed previously 29 and in the present study, which may have resulted from different methods of detection, both studies indicate that ECSODR213G indeed binds to collagen type I.	bind
28469	1	7532	5	13	NULL	NULL	NULL	VLDL	GP		bind					VLDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1470_s_117	12231568	29 In consideration of the repeated observation that apoC-I interferes with the binding of VLDL to the VLDL receptor (apoE mediated) but not with the binding of VLDL to the LDL receptor (apoB-100 mediated), 30 the mechanism of the protection against obesity in the setting of high levels of apoC-I and in the setting of absent VLDL receptor could be similar.	bind
28470	3	7532	5	13	NULL	NULL	NULL	apoC-I	GP		interferes with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1470_s_117	12231568	29 In consideration of the repeated observation that apoC-I interferes with the binding of VLDL to the VLDL receptor (apoE mediated) but not with the binding of VLDL to the LDL receptor (apoB-100 mediated), 30 the mechanism of the protection against obesity in the setting of high levels of apoC-I and in the setting of absent VLDL receptor could be similar.	bind
28471	2	7532	5	13	NULL	NULL	NULL	apoE	GP		mediate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1470_s_117	12231568	29 In consideration of the repeated observation that apoC-I interferes with the binding of VLDL to the VLDL receptor (apoE mediated) but not with the binding of VLDL to the LDL receptor (apoB-100 mediated), 30 the mechanism of the protection against obesity in the setting of high levels of apoC-I and in the setting of absent VLDL receptor could be similar.	bind
28478	4	7532	5	13	NULL	NULL	NULL	apoB-100	GP		mediate					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1470_s_117	12231568	29 In consideration of the repeated observation that apoC-I interferes with the binding of VLDL to the VLDL receptor (apoE mediated) but not with the binding of VLDL to the LDL receptor (apoB-100 mediated), 30 the mechanism of the protection against obesity in the setting of high levels of apoC-I and in the setting of absent VLDL receptor could be similar.	bind
28479	5	7532	5	13	NULL	NULL	NULL	apoC-I	GP		does not interfere with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1470_s_117	12231568	29 In consideration of the repeated observation that apoC-I interferes with the binding of VLDL to the VLDL receptor (apoE mediated) but not with the binding of VLDL to the LDL receptor (apoB-100 mediated), 30 the mechanism of the protection against obesity in the setting of high levels of apoC-I and in the setting of absent VLDL receptor could be similar.	bind
54540	6	7532	5	13	NULL	NULL	NULL	VLDL	GP		bind					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1470_s_117	12231568	29 In consideration of the repeated observation that apoC-I interferes with the binding of VLDL to the VLDL receptor (apoE mediated) but not with the binding of VLDL to the LDL receptor (apoB-100 mediated), 30 the mechanism of the protection against obesity in the setting of high levels of apoC-I and in the setting of absent VLDL receptor could be similar.	bind
30917	1	7532	7	NULL	NULL	0	NULL	VLDL	NULL		binds	NULL				VLDL receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1470_s_117	12231568	29 In consideration of the repeated observation that apoC-I interferes with the binding of VLDL to the VLDL receptor (apoE mediated) but not with the binding of VLDL to the LDL receptor (apoB-100 mediated), 30 the mechanism of the protection against obesity in the setting of high levels of apoC-I and in the setting of absent VLDL receptor could be similar.	bind
30918	2	7532	7	NULL	NULL	0	NULL	apoE	NULL		mediates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1470_s_117	12231568	29 In consideration of the repeated observation that apoC-I interferes with the binding of VLDL to the VLDL receptor (apoE mediated) but not with the binding of VLDL to the LDL receptor (apoB-100 mediated), 30 the mechanism of the protection against obesity in the setting of high levels of apoC-I and in the setting of absent VLDL receptor could be similar.	bind
30919	3	7532	7	NULL	NULL	0	NULL	apoC-I	NULL		interferes with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1470_s_117	12231568	29 In consideration of the repeated observation that apoC-I interferes with the binding of VLDL to the VLDL receptor (apoE mediated) but not with the binding of VLDL to the LDL receptor (apoB-100 mediated), 30 the mechanism of the protection against obesity in the setting of high levels of apoC-I and in the setting of absent VLDL receptor could be similar.	bind
30920	4	7532	7	NULL	NULL	0	NULL	VLDL	NULL		binds	NULL				LDL receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1470_s_117	12231568	29 In consideration of the repeated observation that apoC-I interferes with the binding of VLDL to the VLDL receptor (apoE mediated) but not with the binding of VLDL to the LDL receptor (apoB-100 mediated), 30 the mechanism of the protection against obesity in the setting of high levels of apoC-I and in the setting of absent VLDL receptor could be similar.	bind
30922	5	7532	7	NULL	NULL	0	NULL	apoB-100	NULL		mediates	NULL				statement 4	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1470_s_117	12231568	29 In consideration of the repeated observation that apoC-I interferes with the binding of VLDL to the VLDL receptor (apoE mediated) but not with the binding of VLDL to the LDL receptor (apoB-100 mediated), 30 the mechanism of the protection against obesity in the setting of high levels of apoC-I and in the setting of absent VLDL receptor could be similar.	bind
30924	6	7532	7	NULL	NULL	0	NULL	apoC-I 	NULL		does not interfere with	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1470_s_117	12231568	29 In consideration of the repeated observation that apoC-I interferes with the binding of VLDL to the VLDL receptor (apoE mediated) but not with the binding of VLDL to the LDL receptor (apoB-100 mediated), 30 the mechanism of the protection against obesity in the setting of high levels of apoC-I and in the setting of absent VLDL receptor could be similar.	bind
28465	1	7534	5	13	NULL	NULL	NULL			deletion of	inhibit				promoter region with AP-1-like site	bFGF	GP	effect of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_5_855_s_188	12006402	29 In the present study, deletion of the promoter region containing an AP-1-like site inhibited the effect of bFGF, and EMSA suggested that fenofibric acid did not inhibit nuclear translocation or DNA binding of the Ets-1-like transcription factor to the PAI-1 promoter.	bind
28466	2	7534	5	13	NULL	NULL	NULL	fenofibric acid	Chemical		does not inhibit					nuclear translocation	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_5_855_s_188	12006402	29 In the present study, deletion of the promoter region containing an AP-1-like site inhibited the effect of bFGF, and EMSA suggested that fenofibric acid did not inhibit nuclear translocation or DNA binding of the Ets-1-like transcription factor to the PAI-1 promoter.	bind
28467	3	7534	5	13	NULL	NULL	NULL	Ets-1-like transcription factor	GP		bind					PAI-1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_5_855_s_188	12006402	29 In the present study, deletion of the promoter region containing an AP-1-like site inhibited the effect of bFGF, and EMSA suggested that fenofibric acid did not inhibit nuclear translocation or DNA binding of the Ets-1-like transcription factor to the PAI-1 promoter.	bind
28468	4	7534	5	13	NULL	NULL	NULL	fenofibric acid	Chemical		does not inhibit					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_5_855_s_188	12006402	29 In the present study, deletion of the promoter region containing an AP-1-like site inhibited the effect of bFGF, and EMSA suggested that fenofibric acid did not inhibit nuclear translocation or DNA binding of the Ets-1-like transcription factor to the PAI-1 promoter.	bind
30927	1	7534	7	NULL	NULL	0	NULL		NULL	deletion of	inhibits	NULL			AP-1-like site promoter region	bFGF	NULL	effect of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_5_855_s_188	12006402	29 In the present study, deletion of the promoter region containing an AP-1-like site inhibited the effect of bFGF, and EMSA suggested that fenofibric acid did not inhibit nuclear translocation or DNA binding of the Ets-1-like transcription factor to the PAI-1 promoter.	bind
30928	2	7534	7	NULL	NULL	0	NULL	Ets-1-like transcription factor 	NULL		bind	NULL				PAI-1	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_5_855_s_188	12006402	29 In the present study, deletion of the promoter region containing an AP-1-like site inhibited the effect of bFGF, and EMSA suggested that fenofibric acid did not inhibit nuclear translocation or DNA binding of the Ets-1-like transcription factor to the PAI-1 promoter.	bind
30929	3	7534	7	NULL	NULL	0	NULL	fenofibric acid	NULL		does not inhibit	NULL				statement 2	NULL	nuclear translocation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_5_855_s_188	12006402	29 In the present study, deletion of the promoter region containing an AP-1-like site inhibited the effect of bFGF, and EMSA suggested that fenofibric acid did not inhibit nuclear translocation or DNA binding of the Ets-1-like transcription factor to the PAI-1 promoter.	bind
30930	4	7534	7	NULL	NULL	0	NULL	fenofibric acid	NULL		does not inhibit	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_5_855_s_188	12006402	29 In the present study, deletion of the promoter region containing an AP-1-like site inhibited the effect of bFGF, and EMSA suggested that fenofibric acid did not inhibit nuclear translocation or DNA binding of the Ets-1-like transcription factor to the PAI-1 promoter.	bind
31549	1	7535	5	13	NULL	NULL	NULL	TNF-alpha	GP	soluble	associates with					p75 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_162_3_933_s_165	12598326	29 The fast association/dissociation kinetics of soluble TNF-alpha with the p75 receptor is thought to create an increase in the local concentration of the cytokine in the proximity of the cell membrane, thus potentially augmenting soluble TNF-alpha binding to the p55 receptor.	bind
31550	2	7535	5	13	NULL	NULL	NULL	TNF-alpha	GP	soluble	dissociates with					p75 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_162_3_933_s_165	12598326	29 The fast association/dissociation kinetics of soluble TNF-alpha with the p75 receptor is thought to create an increase in the local concentration of the cytokine in the proximity of the cell membrane, thus potentially augmenting soluble TNF-alpha binding to the p55 receptor.	bind
31551	3	7535	5	13	NULL	NULL	NULL	statement 6	Process	kinetics of	increases					cytokine	GP	local concentration of			NULL	proximity of cell membrane	NULL	NULL	NULL	NULL	gw60_amjpathol_162_3_933_s_165	12598326	29 The fast association/dissociation kinetics of soluble TNF-alpha with the p75 receptor is thought to create an increase in the local concentration of the cytokine in the proximity of the cell membrane, thus potentially augmenting soluble TNF-alpha binding to the p55 receptor.	bind
31552	4	7535	5	13	NULL	NULL	NULL	TNF-alpha	GP		bind					p55 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_162_3_933_s_165	12598326	29 The fast association/dissociation kinetics of soluble TNF-alpha with the p75 receptor is thought to create an increase in the local concentration of the cytokine in the proximity of the cell membrane, thus potentially augmenting soluble TNF-alpha binding to the p55 receptor.	bind
31553	5	7535	5	13	NULL	NULL	NULL	statement 3	Process		augments		potentially			statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_162_3_933_s_165	12598326	29 The fast association/dissociation kinetics of soluble TNF-alpha with the p75 receptor is thought to create an increase in the local concentration of the cytokine in the proximity of the cell membrane, thus potentially augmenting soluble TNF-alpha binding to the p55 receptor.	bind
54541	6	7535	5	13	NULL	NULL	NULL	statement 1	Process		occurs along with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_162_3_933_s_165	12598326	29 The fast association/dissociation kinetics of soluble TNF-alpha with the p75 receptor is thought to create an increase in the local concentration of the cytokine in the proximity of the cell membrane, thus potentially augmenting soluble TNF-alpha binding to the p55 receptor.	bind
30934	1	7535	7	NULL	NULL	0	NULL	TNF-alpha	NULL	soluble	associate with	NULL				p75 receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_162_3_933_s_165	12598326	29 The fast association/dissociation kinetics of soluble TNF-alpha with the p75 receptor is thought to create an increase in the local concentration of the cytokine in the proximity of the cell membrane, thus potentially augmenting soluble TNF-alpha binding to the p55 receptor.	bind
30935	3	7535	7	10	NULL	0	NULL	statement 6		kinetics of	increase					cytokine		local concentration of			NULL	proximity of cell membrane	NULL	NULL	NULL	NULL	gw60_amjpathol_162_3_933_s_165	12598326	29 The fast association/dissociation kinetics of soluble TNF-alpha with the p75 receptor is thought to create an increase in the local concentration of the cytokine in the proximity of the cell membrane, thus potentially augmenting soluble TNF-alpha binding to the p55 receptor.	bind
30937	2	7535	7	10	NULL	0	NULL	TNF-alpha		soluble	dissociates with					p75 receptor					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_162_3_933_s_165	12598326	29 The fast association/dissociation kinetics of soluble TNF-alpha with the p75 receptor is thought to create an increase in the local concentration of the cytokine in the proximity of the cell membrane, thus potentially augmenting soluble TNF-alpha binding to the p55 receptor.	bind
30941	4	7535	7	NULL	NULL	0	NULL	TNF-alpha	NULL	soluble	binds	NULL				p55 receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_162_3_933_s_165	12598326	29 The fast association/dissociation kinetics of soluble TNF-alpha with the p75 receptor is thought to create an increase in the local concentration of the cytokine in the proximity of the cell membrane, thus potentially augmenting soluble TNF-alpha binding to the p55 receptor.	bind
30943	5	7535	7	NULL	NULL	0	NULL	statement 2	NULL		augments	NULL	potentially			statement 4	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_162_3_933_s_165	12598326	29 The fast association/dissociation kinetics of soluble TNF-alpha with the p75 receptor is thought to create an increase in the local concentration of the cytokine in the proximity of the cell membrane, thus potentially augmenting soluble TNF-alpha binding to the p55 receptor.	bind
54542	6	7535	7	10	NULL	0	NULL	statement 1			occurs along with					statement 2					NULL		0	NULL	NULL	NULL	gw60_amjpathol_162_3_933_s_165	12598326	29 The fast association/dissociation kinetics of soluble TNF-alpha with the p75 receptor is thought to create an increase in the local concentration of the cytokine in the proximity of the cell membrane, thus potentially augmenting soluble TNF-alpha binding to the p55 receptor.	bind
28482	1	7536	5	13	NULL	NULL	NULL	estrogen	Chemical	consensus sites for	is present in					betaine homocysteine methyltransferase gene	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_301_s_142	14699020	29 The presence of consensus sites for steroid hormones, including estrogen and androgen binding sites, in the human betaine homocysteine methyltransferase gene 30 may represent a molecular basis of sex steroid effects on plasma betaine.	bind
28483	2	7536	5	13	NULL	NULL	NULL	androgen	Chemical	consensus sites for	is present in					betaine homocysteine methyltransferase gene	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_301_s_142	14699020	29 The presence of consensus sites for steroid hormones, including estrogen and androgen binding sites, in the human betaine homocysteine methyltransferase gene 30 may represent a molecular basis of sex steroid effects on plasma betaine.	bind
28484	3	7536	5	13	NULL	NULL	NULL	estrogen	Chemical		is a type of					steroid hormone	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_301_s_142	14699020	29 The presence of consensus sites for steroid hormones, including estrogen and androgen binding sites, in the human betaine homocysteine methyltransferase gene 30 may represent a molecular basis of sex steroid effects on plasma betaine.	bind
28485	4	7536	5	13	NULL	NULL	NULL	androgen	Chemical		is a type of					steroid hormone	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_301_s_142	14699020	29 The presence of consensus sites for steroid hormones, including estrogen and androgen binding sites, in the human betaine homocysteine methyltransferase gene 30 may represent a molecular basis of sex steroid effects on plasma betaine.	bind
28486	5	7536	5	13	NULL	NULL	NULL	sex steroid	Chemical		effects					betaine	Chemical	plasma			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_301_s_142	14699020	29 The presence of consensus sites for steroid hormones, including estrogen and androgen binding sites, in the human betaine homocysteine methyltransferase gene 30 may represent a molecular basis of sex steroid effects on plasma betaine.	bind
28487	6	7536	5	13	NULL	NULL	NULL	statement 1	Process		represents		may			statement 5	Process	molecular basis of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_301_s_142	14699020	29 The presence of consensus sites for steroid hormones, including estrogen and androgen binding sites, in the human betaine homocysteine methyltransferase gene 30 may represent a molecular basis of sex steroid effects on plasma betaine.	bind
28488	7	7536	5	13	NULL	NULL	NULL	statement 2	Process		represents		may			statement 5	Process	molecular basis of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_301_s_142	14699020	29 The presence of consensus sites for steroid hormones, including estrogen and androgen binding sites, in the human betaine homocysteine methyltransferase gene 30 may represent a molecular basis of sex steroid effects on plasma betaine.	bind
30946	1	7536	7	NULL	NULL	0	NULL	betaine homocysteine methyltransferase gene	NULL	human	consist of	NULL					NULL			estrogen binding site	NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_301_s_142	14699020	29 The presence of consensus sites for steroid hormones, including estrogen and androgen binding sites, in the human betaine homocysteine methyltransferase gene 30 may represent a molecular basis of sex steroid effects on plasma betaine.	bind
30947	2	7536	7	NULL	NULL	0	NULL	betaine homocysteine methyltransferase gene	NULL	human	consist of	NULL					NULL			androgen binding site	NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_301_s_142	14699020	29 The presence of consensus sites for steroid hormones, including estrogen and androgen binding sites, in the human betaine homocysteine methyltransferase gene 30 may represent a molecular basis of sex steroid effects on plasma betaine.	bind
30954	3	7536	7	10	NULL	0	NULL	sex steroid			affects					betaine		plasma			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_301_s_142	14699020	29 The presence of consensus sites for steroid hormones, including estrogen and androgen binding sites, in the human betaine homocysteine methyltransferase gene 30 may represent a molecular basis of sex steroid effects on plasma betaine.	bind
30955	5	7536	7	10	NULL	0	NULL	statement 1	NULL		represents	NULL				statement 3	NULL	molecular basis of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_301_s_142	14699020	29 The presence of consensus sites for steroid hormones, including estrogen and androgen binding sites, in the human betaine homocysteine methyltransferase gene 30 may represent a molecular basis of sex steroid effects on plasma betaine.	bind
46656	4	7536	7	10	NULL	0	NULL	statement 2	NULL		represents	NULL				statement 3	NULL	molecular basis of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_301_s_142	14699020	29 The presence of consensus sites for steroid hormones, including estrogen and androgen binding sites, in the human betaine homocysteine methyltransferase gene 30 may represent a molecular basis of sex steroid effects on plasma betaine.	bind
54543	6	7536	7	10	NULL	0	NULL	estrogen			is a type of					steroid hormone					NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_301_s_142	14699020	29 The presence of consensus sites for steroid hormones, including estrogen and androgen binding sites, in the human betaine homocysteine methyltransferase gene 30 may represent a molecular basis of sex steroid effects on plasma betaine.	bind
54544	7	7536	7	10	NULL	0	NULL	androgen			is a type of					steroid hormone					NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_2_301_s_142	14699020	29 The presence of consensus sites for steroid hormones, including estrogen and androgen binding sites, in the human betaine homocysteine methyltransferase gene 30 may represent a molecular basis of sex steroid effects on plasma betaine.	bind
28489	1	7537	5	13	NULL	NULL	NULL	c-Src	GP		bind		specifically;;directly	SH2 domain		EGFR	GP	activated			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_12_8335_s_267	10075741	29,  49, and  50) demonstrate that the c-Src SH2 domain can bind activated EGFR specifically and directly, suggesting that recruitment of other tyrosine kinases is not necessary to mediate the phosphorylation of Tyr845.	bind
28490	2	7537	5	13	NULL	NULL	NULL	tyrosine kinases	GP	recruitment of 	is not necessary to							mediate phosphorylation of 	Tyr845		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_12_8335_s_267	10075741	29,  49, and  50) demonstrate that the c-Src SH2 domain can bind activated EGFR specifically and directly, suggesting that recruitment of other tyrosine kinases is not necessary to mediate the phosphorylation of Tyr845.	bind
30957	1	7537	7	NULL	NULL	0	NULL	c-Src	NULL		bind	NULL	directly;;specifically	SH2 domain		EGFR	NULL	activated			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_12_8335_s_267	10075741	29,  49, and  50) demonstrate that the c-Src SH2 domain can bind activated EGFR specifically and directly, suggesting that recruitment of other tyrosine kinases is not necessary to mediate the phosphorylation of Tyr845.	bind
30959	2	7537	7	NULL	NULL	0	NULL	tyrosine kinases	NULL	recruitment of	does not mediate	NULL					NULL	phosphorylation of	Tyr845		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_12_8335_s_267	10075741	29,  49, and  50) demonstrate that the c-Src SH2 domain can bind activated EGFR specifically and directly, suggesting that recruitment of other tyrosine kinases is not necessary to mediate the phosphorylation of Tyr845.	bind
30962	3	7537	7	NULL	NULL	0	NULL	statement 1	NULL		suggests	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_12_8335_s_267	10075741	29,  49, and  50) demonstrate that the c-Src SH2 domain can bind activated EGFR specifically and directly, suggesting that recruitment of other tyrosine kinases is not necessary to mediate the phosphorylation of Tyr845.	bind
28491	1	7538	5	13	NULL	NULL	NULL	c-src	GP		bind					SHP-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_5_1367_s_23	10329590	29, 30, 34  hosphorylation of these tyrosine residues mediates binding of c-src and the phosphatase SHP-2, which have been implicated in mediating a variety of signaling events.	bind
28492	2	7538	5	13	NULL	NULL	NULL	SHP-2	GP		is a type of					phosphatase	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_5_1367_s_23	10329590	29, 30, 34  hosphorylation of these tyrosine residues mediates binding of c-src and the phosphatase SHP-2, which have been implicated in mediating a variety of signaling events.	bind
28493	3	7538	5	13	NULL	NULL	NULL			phosphorylation of	mediate			tyrosine residues		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_5_1367_s_23	10329590	29, 30, 34  hosphorylation of these tyrosine residues mediates binding of c-src and the phosphatase SHP-2, which have been implicated in mediating a variety of signaling events.	bind
28494	4	7538	5	13	NULL	NULL	NULL	statement 1	Process		mediate					signaling events	Process	variety of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_5_1367_s_23	10329590	29, 30, 34  hosphorylation of these tyrosine residues mediates binding of c-src and the phosphatase SHP-2, which have been implicated in mediating a variety of signaling events.	bind
30967	1	7538	7	NULL	NULL	0	NULL	 c-src	NULL		bind	NULL				SHP-2	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_5_1367_s_23	10329590	29, 30, 34  hosphorylation of these tyrosine residues mediates binding of c-src and the phosphatase SHP-2, which have been implicated in mediating a variety of signaling events.	bind
30969	2	7538	7	NULL	NULL	0	NULL		NULL	phosphorylation of	mediates	NULL		tyrosine residues		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_5_1367_s_23	10329590	29, 30, 34  hosphorylation of these tyrosine residues mediates binding of c-src and the phosphatase SHP-2, which have been implicated in mediating a variety of signaling events.	bind
30970	3	7538	7	NULL	NULL	0	NULL	SHP-2	NULL		is a type of	NULL				phosphatase	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_5_1367_s_23	10329590	29, 30, 34  hosphorylation of these tyrosine residues mediates binding of c-src and the phosphatase SHP-2, which have been implicated in mediating a variety of signaling events.	bind
30972	4	7538	7	NULL	NULL	0	NULL	statement 1	NULL		mediates	NULL				signaling events	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_5_1367_s_23	10329590	29, 30, 34  hosphorylation of these tyrosine residues mediates binding of c-src and the phosphatase SHP-2, which have been implicated in mediating a variety of signaling events.	bind
28495	1	7539	5	13	NULL	NULL	NULL	C/EBPbeta	GP		bind					CRP	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_5_904_s_77	15731497	29,30  p50 enhanced and stabilized the binding of C/EBPbeta to the CRP promoter and p50 and C/EBPbeta binding sites in the promoter were necessary for full induction of the gene.	bind
28496	2	7539	5	13	NULL	NULL	NULL	p50	GP		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_5_904_s_77	15731497	29,30  p50 enhanced and stabilized the binding of C/EBPbeta to the CRP promoter and p50 and C/EBPbeta binding sites in the promoter were necessary for full induction of the gene.	bind
28497	3	7539	5	13	NULL	NULL	NULL	p50	GP		stabilizes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_5_904_s_77	15731497	29,30  p50 enhanced and stabilized the binding of C/EBPbeta to the CRP promoter and p50 and C/EBPbeta binding sites in the promoter were necessary for full induction of the gene.	bind
28498	4	7539	5	13	NULL	NULL	NULL	CRP	GP		is necessary for				C/EBPbeta binding sites in promoter	CRP gene	GP	full induction of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_5_904_s_77	15731497	29,30  p50 enhanced and stabilized the binding of C/EBPbeta to the CRP promoter and p50 and C/EBPbeta binding sites in the promoter were necessary for full induction of the gene.	bind
28499	5	7539	5	13	NULL	NULL	NULL	CRP	GP		is necessary for				p50 binding sites in promoter	CRP gene	GP	full induction of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_5_904_s_77	15731497	29,30  p50 enhanced and stabilized the binding of C/EBPbeta to the CRP promoter and p50 and C/EBPbeta binding sites in the promoter were necessary for full induction of the gene.	bind
30975	1	7539	7	NULL	NULL	0	NULL	C/EBPbeta	NULL		binds to	NULL				CRP 	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_5_904_s_77	15731497	29,30  p50 enhanced and stabilized the binding of C/EBPbeta to the CRP promoter and p50 and C/EBPbeta binding sites in the promoter were necessary for full induction of the gene.	bind
30976	2	7539	7	NULL	NULL	0	NULL	p50	NULL		enhance	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_5_904_s_77	15731497	29,30  p50 enhanced and stabilized the binding of C/EBPbeta to the CRP promoter and p50 and C/EBPbeta binding sites in the promoter were necessary for full induction of the gene.	bind
30977	3	7539	7	NULL	NULL	0	NULL	p50	NULL		stabilize	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_5_904_s_77	15731497	29,30  p50 enhanced and stabilized the binding of C/EBPbeta to the CRP promoter and p50 and C/EBPbeta binding sites in the promoter were necessary for full induction of the gene.	bind
30978	4	7539	7	NULL	NULL	0	NULL		NULL		is necessary for	NULL			p50 binding site	CRP gene	NULL	full induction of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_5_904_s_77	15731497	29,30  p50 enhanced and stabilized the binding of C/EBPbeta to the CRP promoter and p50 and C/EBPbeta binding sites in the promoter were necessary for full induction of the gene.	bind
30979	5	7539	7	NULL	NULL	0	NULL		NULL		is necessary for	NULL			C/EBPbeta binding site	CRP gene	NULL	full induction of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_5_904_s_77	15731497	29,30  p50 enhanced and stabilized the binding of C/EBPbeta to the CRP promoter and p50 and C/EBPbeta binding sites in the promoter were necessary for full induction of the gene.	bind
28500	1	7540	5	13	NULL	NULL	NULL	annexin V	GP		bind					PS	Chemical				NULL	on the surface of a Ca2+ ionophore-stimulated cell	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_456_s_61	16397140	29,32 - 35     Furthermore, the binding of annexin V to PS on the surface of a Ca2+ ionophore-stimulated cell inhibits the expression of decrypted TF PCA. 23 Therefore, the loss of PS asymmetry appears to be connected to the process of TF decryption.	bind
28501	2	7540	5	13	NULL	NULL	NULL	statement 1	Process		inhibit					TF PCA	Process	expression of;;decrypted			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_456_s_61	16397140	29,32 - 35     Furthermore, the binding of annexin V to PS on the surface of a Ca2+ ionophore-stimulated cell inhibits the expression of decrypted TF PCA. 23 Therefore, the loss of PS asymmetry appears to be connected to the process of TF decryption.	bind
28502	3	7540	5	13	NULL	NULL	NULL	PS asymmetry	Process	loss of	is connected to		appears			TF decryption	Process	process of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_456_s_61	16397140	29,32 - 35     Furthermore, the binding of annexin V to PS on the surface of a Ca2+ ionophore-stimulated cell inhibits the expression of decrypted TF PCA. 23 Therefore, the loss of PS asymmetry appears to be connected to the process of TF decryption.	bind
30980	1	7540	7	NULL	NULL	0	NULL	annexin V	NULL		binds to	NULL				PS	NULL				NULL	surface of a Ca2+ ionophore-stimulated cell	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_456_s_61	16397140	29,32 - 35     Furthermore, the binding of annexin V to PS on the surface of a Ca2+ ionophore-stimulated cell inhibits the expression of decrypted TF PCA. 23 Therefore, the loss of PS asymmetry appears to be connected to the process of TF decryption.	bind
30981	2	7540	7	NULL	NULL	0	NULL	Ca2+ ionophore	NULL		stimulates	NULL				cell	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_456_s_61	16397140	29,32 - 35     Furthermore, the binding of annexin V to PS on the surface of a Ca2+ ionophore-stimulated cell inhibits the expression of decrypted TF PCA. 23 Therefore, the loss of PS asymmetry appears to be connected to the process of TF decryption.	bind
30982	3	7540	7	10	NULL	0	NULL	statement 1			inhibits					TF PCA		expression of;;decrypted			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_456_s_61	16397140	29,32 - 35     Furthermore, the binding of annexin V to PS on the surface of a Ca2+ ionophore-stimulated cell inhibits the expression of decrypted TF PCA. 23 Therefore, the loss of PS asymmetry appears to be connected to the process of TF decryption.	bind
30984	4	7540	7	NULL	NULL	0	NULL	PS asymmetry	NULL	loss of	is connected to	NULL				TF decryption	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_456_s_61	16397140	29,32 - 35     Furthermore, the binding of annexin V to PS on the surface of a Ca2+ ionophore-stimulated cell inhibits the expression of decrypted TF PCA. 23 Therefore, the loss of PS asymmetry appears to be connected to the process of TF decryption.	bind
28503	1	7541	5	13	NULL	NULL	NULL				bind		high affinity	nebulin repeats		actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_67	14976140	29,34  The nebulin repeats bind actin with high affinity, but there is also evidence that nebulette motifs bind troponin T and tropomyosin.	bind
28504	2	7541	5	13	NULL	NULL	NULL				bind			nebulette motifs		troponin T	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_67	14976140	29,34  The nebulin repeats bind actin with high affinity, but there is also evidence that nebulette motifs bind troponin T and tropomyosin.	bind
28505	3	7541	5	13	NULL	NULL	NULL				bind			nebulette motifs		tropomyosin	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_67	14976140	29,34  The nebulin repeats bind actin with high affinity, but there is also evidence that nebulette motifs bind troponin T and tropomyosin.	bind
30985	1	7541	7	NULL	NULL	0	NULL		NULL		bind	NULL	high affinity	nebulin repeats		actin	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_67	14976140	29,34  The nebulin repeats bind actin with high affinity, but there is also evidence that nebulette motifs bind troponin T and tropomyosin.	bind
30986	2	7541	7	NULL	NULL	0	NULL		NULL		bind	NULL		nebulette motifs		troponin T	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_67	14976140	29,34  The nebulin repeats bind actin with high affinity, but there is also evidence that nebulette motifs bind troponin T and tropomyosin.	bind
30987	3	7541	7	NULL	NULL	0	NULL		NULL		bind	NULL		nebulette motifs		tropomyosin	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_67	14976140	29,34  The nebulin repeats bind actin with high affinity, but there is also evidence that nebulette motifs bind troponin T and tropomyosin.	bind
28507	1	7542	5	13	NULL	NULL	NULL	Platelet P-selectin	GP		bind					PSGL-1	GP				NULL	on neutrophils	NULL	NULL	NULL	NULL	gw70_circulation_110_17_2713_s_200	15492312	29,40  Platelet P-selectin binding to PSGL-1 on neutrophils mediates initial tethering, followed by their firm adhesion dependent on CD11b/CD18 (Mac-1) binding to GPIbalpha 41 and/or junctional adhesion molecule-3.	bind
28508	2	7542	5	13	NULL	NULL	NULL	statement 1	Process		mediate					tethering	Process	initial			NULL	neutrophils	NULL	NULL	NULL	NULL	gw70_circulation_110_17_2713_s_200	15492312	29,40  Platelet P-selectin binding to PSGL-1 on neutrophils mediates initial tethering, followed by their firm adhesion dependent on CD11b/CD18 (Mac-1) binding to GPIbalpha 41 and/or junctional adhesion molecule-3.	bind
28509	3	7542	5	13	NULL	NULL	NULL	Mac-1	GP		is					CD11b/CD18	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_17_2713_s_200	15492312	29,40  Platelet P-selectin binding to PSGL-1 on neutrophils mediates initial tethering, followed by their firm adhesion dependent on CD11b/CD18 (Mac-1) binding to GPIbalpha 41 and/or junctional adhesion molecule-3.	bind
28510	4	7542	5	13	NULL	NULL	NULL	Mac-1	GP		bind					GPIbalpha 41	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_17_2713_s_200	15492312	29,40  Platelet P-selectin binding to PSGL-1 on neutrophils mediates initial tethering, followed by their firm adhesion dependent on CD11b/CD18 (Mac-1) binding to GPIbalpha 41 and/or junctional adhesion molecule-3.	bind
28511	5	7542	5	13	NULL	NULL	NULL	Mac-1	GP		bind					junctional adhesion molecule-3	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_17_2713_s_200	15492312	29,40  Platelet P-selectin binding to PSGL-1 on neutrophils mediates initial tethering, followed by their firm adhesion dependent on CD11b/CD18 (Mac-1) binding to GPIbalpha 41 and/or junctional adhesion molecule-3.	bind
28512	6	7542	5	13	NULL	NULL	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_17_2713_s_200	15492312	29,40  Platelet P-selectin binding to PSGL-1 on neutrophils mediates initial tethering, followed by their firm adhesion dependent on CD11b/CD18 (Mac-1) binding to GPIbalpha 41 and/or junctional adhesion molecule-3.	bind
28514	7	7542	5	13	NULL	NULL	NULL	statement 1	Process		is followed by					adhesion	Process	firm			NULL	neutrophils	NULL	NULL	NULL	NULL	gw70_circulation_110_17_2713_s_200	15492312	29,40  Platelet P-selectin binding to PSGL-1 on neutrophils mediates initial tethering, followed by their firm adhesion dependent on CD11b/CD18 (Mac-1) binding to GPIbalpha 41 and/or junctional adhesion molecule-3.	bind
28515	8	7542	5	13	NULL	NULL	NULL	adhesion	Process	firm	is dependent on					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_17_2713_s_200	15492312	29,40  Platelet P-selectin binding to PSGL-1 on neutrophils mediates initial tethering, followed by their firm adhesion dependent on CD11b/CD18 (Mac-1) binding to GPIbalpha 41 and/or junctional adhesion molecule-3.	bind
28516	9	7542	5	13	NULL	NULL	NULL	adhesion	Process	firm	is dependent on					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_17_2713_s_200	15492312	29,40  Platelet P-selectin binding to PSGL-1 on neutrophils mediates initial tethering, followed by their firm adhesion dependent on CD11b/CD18 (Mac-1) binding to GPIbalpha 41 and/or junctional adhesion molecule-3.	bind
28517	10	7542	5	13	NULL	NULL	NULL	statement 8	Process		is an alternative to					statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_17_2713_s_200	15492312	29,40  Platelet P-selectin binding to PSGL-1 on neutrophils mediates initial tethering, followed by their firm adhesion dependent on CD11b/CD18 (Mac-1) binding to GPIbalpha 41 and/or junctional adhesion molecule-3.	bind
30990	1	7542	7	NULL	NULL	0	NULL	Platelet P-selectin	NULL		binds	NULL				PSGL-1 	NULL				NULL	neutrophils	0	NULL	NULL	NULL	gw70_circulation_110_17_2713_s_200	15492312	29,40  Platelet P-selectin binding to PSGL-1 on neutrophils mediates initial tethering, followed by their firm adhesion dependent on CD11b/CD18 (Mac-1) binding to GPIbalpha 41 and/or junctional adhesion molecule-3.	bind
30993	2	7542	7	NULL	NULL	0	NULL	statement 1	NULL		mediates	NULL				initial tethering	NULL				NULL	neutrophils	NULL	NULL	NULL	NULL	gw70_circulation_110_17_2713_s_200	15492312	29,40  Platelet P-selectin binding to PSGL-1 on neutrophils mediates initial tethering, followed by their firm adhesion dependent on CD11b/CD18 (Mac-1) binding to GPIbalpha 41 and/or junctional adhesion molecule-3.	bind
30995	3	7542	7	NULL	NULL	0	NULL	CD11b/CD18 (Mac-1)	NULL		binds to	NULL				GPIbalpha 41 	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_110_17_2713_s_200	15492312	29,40  Platelet P-selectin binding to PSGL-1 on neutrophils mediates initial tethering, followed by their firm adhesion dependent on CD11b/CD18 (Mac-1) binding to GPIbalpha 41 and/or junctional adhesion molecule-3.	bind
30997	4	7542	7	NULL	NULL	0	NULL	CD11b/CD18 (Mac-1)	NULL		binds to	NULL				junctional adhesion molecule-3	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_110_17_2713_s_200	15492312	29,40  Platelet P-selectin binding to PSGL-1 on neutrophils mediates initial tethering, followed by their firm adhesion dependent on CD11b/CD18 (Mac-1) binding to GPIbalpha 41 and/or junctional adhesion molecule-3.	bind
31000	5	7542	7	NULL	NULL	0	NULL	statement 3	NULL		is an alternative to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_110_17_2713_s_200	15492312	29,40  Platelet P-selectin binding to PSGL-1 on neutrophils mediates initial tethering, followed by their firm adhesion dependent on CD11b/CD18 (Mac-1) binding to GPIbalpha 41 and/or junctional adhesion molecule-3.	bind
31003	6	7542	7	10	NULL	0	NULL	statement 1			mediates					adhesion		firm			NULL	neutrophils	NULL	NULL	NULL	NULL	gw70_circulation_110_17_2713_s_200	15492312	29,40  Platelet P-selectin binding to PSGL-1 on neutrophils mediates initial tethering, followed by their firm adhesion dependent on CD11b/CD18 (Mac-1) binding to GPIbalpha 41 and/or junctional adhesion molecule-3.	bind
31004	7	7542	7	NULL	NULL	0	NULL	statement 6	NULL		depends on	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_110_17_2713_s_200	15492312	29,40  Platelet P-selectin binding to PSGL-1 on neutrophils mediates initial tethering, followed by their firm adhesion dependent on CD11b/CD18 (Mac-1) binding to GPIbalpha 41 and/or junctional adhesion molecule-3.	bind
31006	8	7542	7	NULL	NULL	0	NULL	statement 6	NULL		depends on	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_110_17_2713_s_200	15492312	29,40  Platelet P-selectin binding to PSGL-1 on neutrophils mediates initial tethering, followed by their firm adhesion dependent on CD11b/CD18 (Mac-1) binding to GPIbalpha 41 and/or junctional adhesion molecule-3.	bind
28520	1	7545	5	13	NULL	NULL	NULL	CTx PnIB	GP		bind					surface receptors	GP				NULL	HEK cells transfected with high affinity alpha7/5HT-3 cDNA	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_7_4889_s_135	10671525	293 HEK cells were transfected with high affinity alpha7/5HT-3 (see text) and mutant alpha7/5HT-3 subunit cDNAs, and binding of CTx PnIB to the resulting surface receptors was determined as described under	bind
31037	1	7545	7	NULL	NULL	0	NULL	CTx PnIB	NULL		bind	NULL				surface receptor	NULL				NULL	HEK cells transfected with high affinity alpha7/5HT-3 cDNA	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_7_4889_s_135	10671525	293 HEK cells were transfected with high affinity alpha7/5HT-3 (see text) and mutant alpha7/5HT-3 subunit cDNAs, and binding of CTx PnIB to the resulting surface receptors was determined as described under	bind
28523	1	7546	5	13	NULL	NULL	NULL	CTx ImI	GP		bind					surface receptors	GP				NULL	HEK cells transfected with high affinity alpha7/5HT-3 cDNA	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_28_19517_s_111	10391883	293 HEK cells were transfected with wild-type and mutant alpha7/5HT-3 subunit cDNAs and binding of CTx ImI to the resulting surface receptors was determined as described under	bind
31040	1	7546	7	NULL	NULL	0	NULL	CTx ImI 	NULL		bind	NULL				surface receptor	NULL				NULL	HEK cells transfected with wild-type alpha7/5HT-3 subunit cDNA	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_28_19517_s_111	10391883	293 HEK cells were transfected with wild-type and mutant alpha7/5HT-3 subunit cDNAs and binding of CTx ImI to the resulting surface receptors was determined as described under	bind
28524	1	7549	5	13	NULL	NULL	NULL	guanine nucleotides	NucleicAcid		bind					G proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_26_20020_s_81	10777492	293T cells expressing GST-tagged G proteins and GEFs were labeled with 32Pi, and guanine nucleotides bound to G proteins were analyzed by TLC.	bind
31047	1	7549	7	10	NULL	0	NULL	guanine nucleotides			bind					G proteins					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_26_20020_s_81	10777492	293T cells expressing GST-tagged G proteins and GEFs were labeled with 32Pi, and guanine nucleotides bound to G proteins were analyzed by TLC.	bind
28526	1	7556	5	13	NULL	NULL	NULL	alphaLacidbeta2base	GP		bind		lesser extent			ICAM-1	GP				NULL	293T transfectants	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_14642_s_235	11279101	293T transfectants that expressed alphaLacidbeta2base showed little binding to ICAM-1, whereas cells expressing wild-type alphaLbeta2 strongly bound to ICAM-1.	bind
28528	2	7556	5	13	NULL	NULL	NULL	alphaLbeta2	GP	wild-type	bind		strongly			ICAM-1	GP				NULL	293T transfectants	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_14642_s_235	11279101	293T transfectants that expressed alphaLacidbeta2base showed little binding to ICAM-1, whereas cells expressing wild-type alphaLbeta2 strongly bound to ICAM-1.	bind
31048	1	7556	7	NULL	NULL	0	NULL	alphaLacidbeta2base	NULL		bind	NULL	less			ICAM-1	NULL				NULL	293T transfectants	0	NULL	NULL	NULL	gw60_jbiolchem_276_18_14642_s_235	11279101	293T transfectants that expressed alphaLacidbeta2base showed little binding to ICAM-1, whereas cells expressing wild-type alphaLbeta2 strongly bound to ICAM-1.	bind
31049	2	7556	7	10	NULL	0	NULL	alphaLbeta2		wild-type	bind		strongly			ICAM-1					NULL	293T transfectants	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_14642_s_235	11279101	293T transfectants that expressed alphaLacidbeta2base showed little binding to ICAM-1, whereas cells expressing wild-type alphaLbeta2 strongly bound to ICAM-1.	bind
28529	1	7557	5	13	NULL	NULL	NULL	MDM2	GP		bind					ARF peptide	GP		N-terminal		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_40583_s_219	11507088	2A10 inhibits the binding between MDM2 and an ARF N-terminal peptide  in vitro ( 8).	bind
28530	2	7557	5	13	NULL	NULL	NULL	2A10	GP		inhibit					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_40583_s_219	11507088	2A10 inhibits the binding between MDM2 and an ARF N-terminal peptide  in vitro ( 8).	bind
31050	1	7557	7	NULL	NULL	0	NULL	MDM2	NULL		bind	NULL				ARF peptide	NULL		N-terminal		NULL	in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_276_44_40583_s_219	11507088	2A10 inhibits the binding between MDM2 and an ARF N-terminal peptide  in vitro ( 8).	bind
31051	2	7557	7	10	NULL	0	NULL	2A10			inhibits					statement 1					NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_40583_s_219	11507088	2A10 inhibits the binding between MDM2 and an ARF N-terminal peptide  in vitro ( 8).	bind
28531	1	7559	5	13	NULL	NULL	NULL	2B4	GP		bind					CD48	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-immunol_170_10_12734329_s_3	12734329	2B4 binds to CD48 and activates NK cytotoxicity, but its function on CD8(+)  T cells is not clear.	bind
28532	2	7559	5	13	NULL	NULL	NULL	statement 1	Process		activates					NK cytotoxicity	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-immunol_170_10_12734329_s_3	12734329	2B4 binds to CD48 and activates NK cytotoxicity, but its function on CD8(+)  T cells is not clear.	bind
31052	1	7559	7	NULL	NULL	0	NULL	2B4	NULL		binds to	NULL				CD48	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-immunol_170_10_12734329_s_3	12734329	2B4 binds to CD48 and activates NK cytotoxicity, but its function on CD8(+)  T cells is not clear.	bind
31053	2	7559	7	NULL	NULL	0	NULL	statement 1	NULL		activates	NULL				NK cytotoxicity	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-immunol_170_10_12734329_s_3	12734329	2B4 binds to CD48 and activates NK cytotoxicity, but its function on CD8(+)  T cells is not clear.	bind
28533	1	7560	5	13	NULL	NULL	NULL	lipoproteins	GP		bind					LDLR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_10_7109_s_30	10702278	2E8 is a monoclonal antibody (mAb) that binds to apoE and prevents apoE-mediated binding of lipoproteins to the LDLR.	bind
28534	2	7560	5	13	NULL	NULL	NULL	apoE	GP		mediate					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_10_7109_s_30	10702278	2E8 is a monoclonal antibody (mAb) that binds to apoE and prevents apoE-mediated binding of lipoproteins to the LDLR.	bind
28535	3	7560	5	13	NULL	NULL	NULL	2E8	GP		is a type of					mAb	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_10_7109_s_30	10702278	2E8 is a monoclonal antibody (mAb) that binds to apoE and prevents apoE-mediated binding of lipoproteins to the LDLR.	bind
28536	4	7560	5	13	NULL	NULL	NULL	mAb	GP		is					monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_10_7109_s_30	10702278	2E8 is a monoclonal antibody (mAb) that binds to apoE and prevents apoE-mediated binding of lipoproteins to the LDLR.	bind
28537	5	7560	5	13	NULL	NULL	NULL	2E8	GP		bind					apoE	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_10_7109_s_30	10702278	2E8 is a monoclonal antibody (mAb) that binds to apoE and prevents apoE-mediated binding of lipoproteins to the LDLR.	bind
28538	6	7560	5	13	NULL	NULL	NULL	statement 5	Process		prevents					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_10_7109_s_30	10702278	2E8 is a monoclonal antibody (mAb) that binds to apoE and prevents apoE-mediated binding of lipoproteins to the LDLR.	bind
31054	1	7560	7	NULL	NULL	0	NULL	2E8	NULL		binds to	NULL				apoE	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_10_7109_s_30	10702278	2E8 is a monoclonal antibody (mAb) that binds to apoE and prevents apoE-mediated binding of lipoproteins to the LDLR.	bind
31055	2	7560	7	NULL	NULL	0	NULL	2E8	NULL		is a type of	NULL				mAb	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_10_7109_s_30	10702278	2E8 is a monoclonal antibody (mAb) that binds to apoE and prevents apoE-mediated binding of lipoproteins to the LDLR.	bind
31056	3	7560	7	NULL	NULL	0	NULL	mAb	NULL		is	NULL				monoclonal antibody	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_10_7109_s_30	10702278	2E8 is a monoclonal antibody (mAb) that binds to apoE and prevents apoE-mediated binding of lipoproteins to the LDLR.	bind
31057	4	7560	7	NULL	NULL	0	NULL	lipoproteins	NULL		bind	NULL				LDLR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_10_7109_s_30	10702278	2E8 is a monoclonal antibody (mAb) that binds to apoE and prevents apoE-mediated binding of lipoproteins to the LDLR.	bind
31058	5	7560	7	NULL	NULL	0	NULL	apoE	NULL		mediates	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_10_7109_s_30	10702278	2E8 is a monoclonal antibody (mAb) that binds to apoE and prevents apoE-mediated binding of lipoproteins to the LDLR.	bind
31059	6	7560	7	NULL	NULL	0	NULL	statement 1	NULL		prevents	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_10_7109_s_30	10702278	2E8 is a monoclonal antibody (mAb) that binds to apoE and prevents apoE-mediated binding of lipoproteins to the LDLR.	bind
28539	1	7561	5	13	NULL	NULL	NULL	2M	GP		bind					growth factor	GP				NULL	AD-DD plasma samples	NULL	NULL	NULL	NULL	gw70_neurobioldis_14_3_504_s_132	14678766	2M in the other AD-DD plasma samples bound growth factor equivalently to the  2M in the II plasma samples.	bind
28540	2	7561	5	13	NULL	NULL	NULL	2M	GP		bind					growth factor	GP				NULL	II plasma samples	NULL	NULL	NULL	NULL	gw70_neurobioldis_14_3_504_s_132	14678766	2M in the other AD-DD plasma samples bound growth factor equivalently to the  2M in the II plasma samples.	bind
28541	3	7561	5	13	NULL	NULL	NULL	statement 1	Process		is equivalent to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_neurobioldis_14_3_504_s_132	14678766	2M in the other AD-DD plasma samples bound growth factor equivalently to the  2M in the II plasma samples.	bind
31060	1	7561	7	10	NULL	0	NULL	2M			bind					growth factor					NULL	AD-DD plasma samples	NULL	NULL	NULL	NULL	gw70_neurobioldis_14_3_504_s_132	14678766	2M in the other AD-DD plasma samples bound growth factor equivalently to the  2M in the II plasma samples.	bind
54559	2	7561	7	10	NULL	0	NULL	2M			bind					growth factor					NULL	II plasma samples	0	NULL	NULL	NULL	gw70_neurobioldis_14_3_504_s_132	14678766	2M in the other AD-DD plasma samples bound growth factor equivalently to the  2M in the II plasma samples.	bind
54560	3	7561	7	10	NULL	0	NULL	statement 1			is equivalent to					statement 2					NULL		0	NULL	NULL	NULL	gw70_neurobioldis_14_3_504_s_132	14678766	2M in the other AD-DD plasma samples bound growth factor equivalently to the  2M in the II plasma samples.	bind
28542	1	7562	5	13	NULL	NULL	NULL	2ME2	Chemical		bind					tubulin	GP		colchicine binding site		NULL		NULL	NULL	NULL	NULL	gw60_cancercell_3_4_363_s_128	12726862	2ME2 has been shown to bind to the colchicine binding site of tubulin  (D'Amato et al., 1994  ) and to depolymerize microtubules in endothelial  (Fotsis et al., 1994  ) as well as in tumor cells  (Aizu-Yokota et al., 1995  ), resulting in mitotic arrest and cell death.	bind
28543	2	7562	5	13	NULL	NULL	NULL	2ME2	Chemical		depolymerize					microtubules	CellComponent				NULL	in endothelial cells	NULL	NULL	NULL	NULL	gw60_cancercell_3_4_363_s_128	12726862	2ME2 has been shown to bind to the colchicine binding site of tubulin  (D'Amato et al., 1994  ) and to depolymerize microtubules in endothelial  (Fotsis et al., 1994  ) as well as in tumor cells  (Aizu-Yokota et al., 1995  ), resulting in mitotic arrest and cell death.	bind
28544	3	7562	5	13	NULL	NULL	NULL	2ME2	Chemical		depolymerize					microtubules	CellComponent				NULL	in tumor cells 	NULL	NULL	NULL	NULL	gw60_cancercell_3_4_363_s_128	12726862	2ME2 has been shown to bind to the colchicine binding site of tubulin  (D'Amato et al., 1994  ) and to depolymerize microtubules in endothelial  (Fotsis et al., 1994  ) as well as in tumor cells  (Aizu-Yokota et al., 1995  ), resulting in mitotic arrest and cell death.	bind
28546	4	7562	5	13	NULL	NULL	NULL	statement 2	Process		results in					mitotic arrest	Process				NULL		NULL	NULL	NULL	NULL	gw60_cancercell_3_4_363_s_128	12726862	2ME2 has been shown to bind to the colchicine binding site of tubulin  (D'Amato et al., 1994  ) and to depolymerize microtubules in endothelial  (Fotsis et al., 1994  ) as well as in tumor cells  (Aizu-Yokota et al., 1995  ), resulting in mitotic arrest and cell death.	bind
28547	5	7562	5	13	NULL	NULL	NULL	statement 2	Process		results in					cell death	Process				NULL		NULL	NULL	NULL	NULL	gw60_cancercell_3_4_363_s_128	12726862	2ME2 has been shown to bind to the colchicine binding site of tubulin  (D'Amato et al., 1994  ) and to depolymerize microtubules in endothelial  (Fotsis et al., 1994  ) as well as in tumor cells  (Aizu-Yokota et al., 1995  ), resulting in mitotic arrest and cell death.	bind
28548	6	7562	5	13	NULL	NULL	NULL	statement 3	Process		results in					mitotic arrest	Process				NULL		NULL	NULL	NULL	NULL	gw60_cancercell_3_4_363_s_128	12726862	2ME2 has been shown to bind to the colchicine binding site of tubulin  (D'Amato et al., 1994  ) and to depolymerize microtubules in endothelial  (Fotsis et al., 1994  ) as well as in tumor cells  (Aizu-Yokota et al., 1995  ), resulting in mitotic arrest and cell death.	bind
28549	7	7562	5	13	NULL	NULL	NULL	statement 3	Process		results in					cell death	Process				NULL		NULL	NULL	NULL	NULL	gw60_cancercell_3_4_363_s_128	12726862	2ME2 has been shown to bind to the colchicine binding site of tubulin  (D'Amato et al., 1994  ) and to depolymerize microtubules in endothelial  (Fotsis et al., 1994  ) as well as in tumor cells  (Aizu-Yokota et al., 1995  ), resulting in mitotic arrest and cell death.	bind
31061	1	7562	7	NULL	NULL	0	NULL	ME2	NULL		bind	NULL				tubulin	NULL		colchicine binding site		NULL		0	NULL	NULL	NULL	gw60_cancercell_3_4_363_s_128	12726862	2ME2 has been shown to bind to the colchicine binding site of tubulin  (D'Amato et al., 1994  ) and to depolymerize microtubules in endothelial  (Fotsis et al., 1994  ) as well as in tumor cells  (Aizu-Yokota et al., 1995  ), resulting in mitotic arrest and cell death.	bind
31062	2	7562	7	NULL	NULL	0	NULL	statement 1	NULL		depolymerize	NULL				microtubules	NULL				NULL	endothelial cells	0	NULL	NULL	NULL	gw60_cancercell_3_4_363_s_128	12726862	2ME2 has been shown to bind to the colchicine binding site of tubulin  (D'Amato et al., 1994  ) and to depolymerize microtubules in endothelial  (Fotsis et al., 1994  ) as well as in tumor cells  (Aizu-Yokota et al., 1995  ), resulting in mitotic arrest and cell death.	bind
31063	3	7562	7	NULL	NULL	0	NULL	statement 1	NULL		depolymerize	NULL				microtubules	NULL				NULL	tumor cells	0	NULL	NULL	NULL	gw60_cancercell_3_4_363_s_128	12726862	2ME2 has been shown to bind to the colchicine binding site of tubulin  (D'Amato et al., 1994  ) and to depolymerize microtubules in endothelial  (Fotsis et al., 1994  ) as well as in tumor cells  (Aizu-Yokota et al., 1995  ), resulting in mitotic arrest and cell death.	bind
31064	4	7562	7	NULL	NULL	0	NULL	statement 2	NULL		results in	NULL				mitotic arrest	NULL				NULL		0	NULL	NULL	NULL	gw60_cancercell_3_4_363_s_128	12726862	2ME2 has been shown to bind to the colchicine binding site of tubulin  (D'Amato et al., 1994  ) and to depolymerize microtubules in endothelial  (Fotsis et al., 1994  ) as well as in tumor cells  (Aizu-Yokota et al., 1995  ), resulting in mitotic arrest and cell death.	bind
31065	5	7562	7	NULL	NULL	0	NULL	statement 3	NULL		results in	NULL				mitotic arrest	NULL				NULL		0	NULL	NULL	NULL	gw60_cancercell_3_4_363_s_128	12726862	2ME2 has been shown to bind to the colchicine binding site of tubulin  (D'Amato et al., 1994  ) and to depolymerize microtubules in endothelial  (Fotsis et al., 1994  ) as well as in tumor cells  (Aizu-Yokota et al., 1995  ), resulting in mitotic arrest and cell death.	bind
31066	6	7562	7	NULL	NULL	0	NULL	statement 4	NULL		leads to	NULL				cell death	NULL				NULL		0	NULL	NULL	NULL	gw60_cancercell_3_4_363_s_128	12726862	2ME2 has been shown to bind to the colchicine binding site of tubulin  (D'Amato et al., 1994  ) and to depolymerize microtubules in endothelial  (Fotsis et al., 1994  ) as well as in tumor cells  (Aizu-Yokota et al., 1995  ), resulting in mitotic arrest and cell death.	bind
31067	7	7562	7	NULL	NULL	0	NULL	statement 5	NULL		leads to	NULL				cell death	NULL				NULL		0	NULL	NULL	NULL	gw60_cancercell_3_4_363_s_128	12726862	2ME2 has been shown to bind to the colchicine binding site of tubulin  (D'Amato et al., 1994  ) and to depolymerize microtubules in endothelial  (Fotsis et al., 1994  ) as well as in tumor cells  (Aizu-Yokota et al., 1995  ), resulting in mitotic arrest and cell death.	bind
28551	1	7563	5	13	NULL	NULL	NULL	NrpR	GP		bind					DNA	NucleicAcid			operator	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_7_5236_s_184	15590692	2OG inhibits binding of NrpR to operator DNA.	bind
28552	2	7563	5	13	NULL	NULL	NULL	2OG	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_7_5236_s_184	15590692	2OG inhibits binding of NrpR to operator DNA.	bind
31068	1	7563	7	NULL	NULL	0	NULL	NrpR	NULL		bind	NULL				DNA	NULL			operator	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_7_5236_s_184	15590692	2OG inhibits binding of NrpR to operator DNA.	bind
31069	2	7563	7	NULL	NULL	0	NULL	OG	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_7_5236_s_184	15590692	2OG inhibits binding of NrpR to operator DNA.	bind
28553	1	7564	5	13	NULL	NULL	NULL	2xTK49	NucleicAcid		bind		specifically		PPE	hnRNP L	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_15_6303_s_262	16024770	2xTK49 PPE specifically binds only hnRNP L.	bind
31070	1	7564	7	10	NULL	0	NULL	TK49 	NULL		binds	NULL	specifically		PPE	hnRNP L	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_15_6303_s_262	16024770	2xTK49 PPE specifically binds only hnRNP L.	bind
28554	1	7565	5	13	NULL	NULL	NULL	RNA	NucleicAcid	multisite binding of	occurs during					 c- src neural-specific splicing	Process	regulation of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_456_s_139	11788707	3       Chou,M.Y., Underwood,J.G., Nikolic,J., Luu,M.H. and Black,D.L. (2000) Multisite RNA binding and release of polypyrimidine tract binding protein during the regulation of c- src neural-specific splicing.	bind
28555	2	7565	5	13	NULL	NULL	NULL	polypyrimidine tract binding protein	Process	release of	occurs during					c- src neural-specific splicing	Process	regulation of 			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_456_s_139	11788707	3       Chou,M.Y., Underwood,J.G., Nikolic,J., Luu,M.H. and Black,D.L. (2000) Multisite RNA binding and release of polypyrimidine tract binding protein during the regulation of c- src neural-specific splicing.	bind
31121	1	7565	7	10	NULL	0	NULL	RNA		multisite binding of	occurs during 					c- src neural-specific splicing		regulation of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_456_s_139	11788707	3       Chou,M.Y., Underwood,J.G., Nikolic,J., Luu,M.H. and Black,D.L. (2000) Multisite RNA binding and release of polypyrimidine tract binding protein during the regulation of c- src neural-specific splicing.	bind
31123	2	7565	7	NULL	NULL	0	NULL	polypyrimidine tract binding protein 	NULL	release of	occurs during	NULL				c- src neural-specific splicing	NULL	regulation of			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_456_s_139	11788707	3       Chou,M.Y., Underwood,J.G., Nikolic,J., Luu,M.H. and Black,D.L. (2000) Multisite RNA binding and release of polypyrimidine tract binding protein during the regulation of c- src neural-specific splicing.	bind
28556	1	7566	5	13	NULL	NULL	NULL	Raf	GP		bind					GST-Ras-GTP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_40_23681_s_289	7559537	3    at  >50-fold molar excess to Raf does not inhibit the binding of Raf to  GST-Ras-GTP ( Fig. 6,  upper panel,  lanes 1  and  2).	bind
31124	1	7566	7	NULL	NULL	0	NULL	Raf 	NULL		bind	NULL				GST-Ras-GTP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_40_23681_s_289	7559537	3    at  >50-fold molar excess to Raf does not inhibit the binding of Raf to  GST-Ras-GTP ( Fig. 6,  upper panel,  lanes 1  and  2).	bind
28558	1	7568	5	13	NULL	NULL	NULL	XRE	GP		bind					AHR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31845_s_342	9395531	3   This relatively mild effect of oxidation on XRE binding of the AHR.	bind
31132	1	7568	7	NULL	NULL	0	NULL	XRE	NULL		bind	NULL				AHR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_50_31845_s_342	9395531	3   This relatively mild effect of oxidation on XRE binding of the AHR.	bind
28657	1	7569	5	13	NULL	NULL	NULL	dystrophin	GP		bind					actin filaments	GP		amino terminus		NULL	cytoplasmic side of the oligomeric complex	NULL	NULL	NULL	NULL	gw60_amjpathol_153_5_1623_s_12	9811355	3  At the cytoplasmic side of the oligomeric complex, dystrophin binds actin filaments along its amino terminus and spectrin-like rod domain.	bind
28658	2	7569	5	13	NULL	NULL	NULL	dystrophin	GP		bind					actin filaments	GP		spectrin-like rod domain		NULL	cytoplasmic side of the oligomeric complex	NULL	NULL	NULL	NULL	gw60_amjpathol_153_5_1623_s_12	9811355	3  At the cytoplasmic side of the oligomeric complex, dystrophin binds actin filaments along its amino terminus and spectrin-like rod domain.	bind
31138	1	7569	7	10	NULL	0	NULL	dystrophin	NULL		binds	NULL				actin filaments	NULL		amino terminus		NULL	cytoplasmic side of the oligomeric complex	NULL	NULL	NULL	NULL	gw60_amjpathol_153_5_1623_s_12	9811355	3  At the cytoplasmic side of the oligomeric complex, dystrophin binds actin filaments along its amino terminus and spectrin-like rod domain.	bind
31139	2	7569	7	NULL	NULL	0	NULL	dystrophin	NULL		binds	NULL				actin filaments	NULL		spectrin-like rod domain		NULL	cytoplasmic side of the oligomeric complex	NULL	NULL	NULL	NULL	gw60_amjpathol_153_5_1623_s_12	9811355	3  At the cytoplasmic side of the oligomeric complex, dystrophin binds actin filaments along its amino terminus and spectrin-like rod domain.	bind
28661	1	7570	5	13	NULL	NULL	NULL	apoB100 gene	GP	point mutation	causes					FDB	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_802_s_28	10073989	3  FDB is a genetic disorder caused by point mutations in the gene encoding for apoB100 that reduces the binding ability of LDL particles to the LDLR; as a consequence, LDL removal is reduced, and affected individuals develop high plasma cholesterol concentrations.	bind
28662	2	7570	5	13	NULL	NULL	NULL	FDB	MedicalFinding		is a type of					genetic disorder	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_802_s_28	10073989	3  FDB is a genetic disorder caused by point mutations in the gene encoding for apoB100 that reduces the binding ability of LDL particles to the LDLR; as a consequence, LDL removal is reduced, and affected individuals develop high plasma cholesterol concentrations.	bind
28663	3	7570	5	13	NULL	NULL	NULL	LDL particles	GP		bind					LDLR	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_802_s_28	10073989	3  FDB is a genetic disorder caused by point mutations in the gene encoding for apoB100 that reduces the binding ability of LDL particles to the LDLR; as a consequence, LDL removal is reduced, and affected individuals develop high plasma cholesterol concentrations.	bind
28664	4	7570	5	13	NULL	NULL	NULL	apoB100 gene	GP	point mutation	reduces					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_802_s_28	10073989	3  FDB is a genetic disorder caused by point mutations in the gene encoding for apoB100 that reduces the binding ability of LDL particles to the LDLR; as a consequence, LDL removal is reduced, and affected individuals develop high plasma cholesterol concentrations.	bind
28665	5	7570	5	13	NULL	NULL	NULL	statement 4	Process		leads to					LDL	GP	reduced removal of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_802_s_28	10073989	3  FDB is a genetic disorder caused by point mutations in the gene encoding for apoB100 that reduces the binding ability of LDL particles to the LDLR; as a consequence, LDL removal is reduced, and affected individuals develop high plasma cholesterol concentrations.	bind
28666	6	7570	5	13	NULL	NULL	NULL	statement 5	Process		leads to					plasma cholesterol	Chemical	high concentration of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_802_s_28	10073989	3  FDB is a genetic disorder caused by point mutations in the gene encoding for apoB100 that reduces the binding ability of LDL particles to the LDLR; as a consequence, LDL removal is reduced, and affected individuals develop high plasma cholesterol concentrations.	bind
31141	1	7570	7	NULL	NULL	0	NULL	FDB	NULL		is a type of	NULL				genetic disorder	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_802_s_28	10073989	3  FDB is a genetic disorder caused by point mutations in the gene encoding for apoB100 that reduces the binding ability of LDL particles to the LDLR; as a consequence, LDL removal is reduced, and affected individuals develop high plasma cholesterol concentrations.	bind
31142	2	7570	7	NULL	NULL	0	NULL	apoB100 gene	NULL	point mutation 	cause	NULL				FDB	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_802_s_28	10073989	3  FDB is a genetic disorder caused by point mutations in the gene encoding for apoB100 that reduces the binding ability of LDL particles to the LDLR; as a consequence, LDL removal is reduced, and affected individuals develop high plasma cholesterol concentrations.	bind
31144	3	7570	7	NULL	NULL	0	NULL	LDL particles	NULL		bind	NULL				LDLR	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_802_s_28	10073989	3  FDB is a genetic disorder caused by point mutations in the gene encoding for apoB100 that reduces the binding ability of LDL particles to the LDLR; as a consequence, LDL removal is reduced, and affected individuals develop high plasma cholesterol concentrations.	bind
31145	4	7570	7	NULL	NULL	0	NULL	apoB100 gene	NULL	point mutation	reduces	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_802_s_28	10073989	3  FDB is a genetic disorder caused by point mutations in the gene encoding for apoB100 that reduces the binding ability of LDL particles to the LDLR; as a consequence, LDL removal is reduced, and affected individuals develop high plasma cholesterol concentrations.	bind
31146	5	7570	7	NULL	NULL	0	NULL	statement 4	NULL		reduce	NULL				LDL	NULL	removal of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_802_s_28	10073989	3  FDB is a genetic disorder caused by point mutations in the gene encoding for apoB100 that reduces the binding ability of LDL particles to the LDLR; as a consequence, LDL removal is reduced, and affected individuals develop high plasma cholesterol concentrations.	bind
31147	6	7570	7	NULL	NULL	0	NULL	statement 5	NULL		leads to	NULL				plasma cholesterol	NULL	high concentration of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_802_s_28	10073989	3  FDB is a genetic disorder caused by point mutations in the gene encoding for apoB100 that reduces the binding ability of LDL particles to the LDLR; as a consequence, LDL removal is reduced, and affected individuals develop high plasma cholesterol concentrations.	bind
28667	1	7572	5	13	NULL	NULL	NULL	SUR1	GP		bind			NBD1		ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_10_873_s_122	11073882	3  It was shown that SUR1 binds ATP at NBD1 and ADP at NBD2.	bind
28668	2	7572	5	13	NULL	NULL	NULL	SUR1	GP		bind			NBD2		ADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_10_873_s_122	11073882	3  It was shown that SUR1 binds ATP at NBD1 and ADP at NBD2.	bind
31195	1	7572	7	NULL	NULL	0	NULL	SUR1 	NULL		binds	NULL		NBD1		ATP	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_10_873_s_122	11073882	3  It was shown that SUR1 binds ATP at NBD1 and ADP at NBD2.	bind
31196	2	7572	7	NULL	NULL	0	NULL	SUR1 	NULL		bind	NULL		NBD2		ADP	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_10_873_s_122	11073882	3  It was shown that SUR1 binds ATP at NBD1 and ADP at NBD2.	bind
28671	1	7574	5	13	NULL	NULL	NULL	fibrinogen	GP		bind					GPIIb-IIIa	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2127_s_16	10595941	3  Subsequent binding of fibrinogen to GPIIb-IIIa promotes platelet aggregation and formation of an effective hemostatic plug at intermediate shear rates.	bind
28672	2	7574	5	13	NULL	NULL	NULL	statement 1	Process		promotes					platelet aggregation	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2127_s_16	10595941	3  Subsequent binding of fibrinogen to GPIIb-IIIa promotes platelet aggregation and formation of an effective hemostatic plug at intermediate shear rates.	bind
28673	3	7574	5	13	NULL	NULL	NULL	statement 1	Process		forms					hemostatic plug					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2127_s_16	10595941	3  Subsequent binding of fibrinogen to GPIIb-IIIa promotes platelet aggregation and formation of an effective hemostatic plug at intermediate shear rates.	bind
28674	4	7574	5	13	NULL	NULL	NULL	statement 3	Process		occurs at					shear rates		intermediate			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2127_s_16	10595941	3  Subsequent binding of fibrinogen to GPIIb-IIIa promotes platelet aggregation and formation of an effective hemostatic plug at intermediate shear rates.	bind
31197	1	7574	7	NULL	NULL	0	NULL	fibrinogen	NULL		binds to	NULL				GPIIb-IIIa	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_6_2127_s_16	10595941	3  Subsequent binding of fibrinogen to GPIIb-IIIa promotes platelet aggregation and formation of an effective hemostatic plug at intermediate shear rates.	bind
31198	2	7574	7	NULL	NULL	0	NULL	statement 1	NULL		promotes	NULL				platelet aggregation	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_6_2127_s_16	10595941	3  Subsequent binding of fibrinogen to GPIIb-IIIa promotes platelet aggregation and formation of an effective hemostatic plug at intermediate shear rates.	bind
31199	3	7574	7	NULL	NULL	0	NULL	statement 1	NULL		forms	NULL				hemostatic plug 	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_6_2127_s_16	10595941	3  Subsequent binding of fibrinogen to GPIIb-IIIa promotes platelet aggregation and formation of an effective hemostatic plug at intermediate shear rates.	bind
28675	1	7575	5	13	NULL	NULL	NULL	TRs	GP		regulate					alpha-MHC gene	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_6_700_s_149	10747007	3  The alpha-MHC gene is transcriptionally regulated by TRs, which bind to a positive TRE in the promoter of the gene.	bind
28676	2	7575	5	13	NULL	NULL	NULL	TRs	GP		bind					alpha-MHC gene	GP			positive TRE in the promoter	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_6_700_s_149	10747007	3  The alpha-MHC gene is transcriptionally regulated by TRs, which bind to a positive TRE in the promoter of the gene.	bind
31200	1	7575	7	NULL	NULL	0	NULL	TRs	NULL		bind	NULL				alpha-MHC gene	NULL			positive TRE in the promoter	NULL		0	NULL	NULL	NULL	gw60_circulationres_86_6_700_s_149	10747007	3  The alpha-MHC gene is transcriptionally regulated by TRs, which bind to a positive TRE in the promoter of the gene.	bind
31201	2	7575	7	NULL	NULL	0	NULL	TRs	NULL		regulate	NULL				alpha-MHC gene	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_86_6_700_s_149	10747007	3  The alpha-MHC gene is transcriptionally regulated by TRs, which bind to a positive TRE in the promoter of the gene.	bind
28677	1	7576	5	13	NULL	NULL	NULL	thrombin	GP		bind					TM	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_10_1292_s_22	8857927	3  Thus, binding of thrombin to TM induces a negative feedback loop that stops the coagulation.	bind
28678	2	7576	5	13	NULL	NULL	NULL	statement 1	Process		induces					negative feedback loop	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_10_1292_s_22	8857927	3  Thus, binding of thrombin to TM induces a negative feedback loop that stops the coagulation.	bind
28679	3	7576	5	13	NULL	NULL	NULL	statement 2	Process		stops					coagulation	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_10_1292_s_22	8857927	3  Thus, binding of thrombin to TM induces a negative feedback loop that stops the coagulation.	bind
31202	1	7576	7	NULL	NULL	0	NULL	thrombin	NULL		binds	NULL				TM	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_10_1292_s_22	8857927	3  Thus, binding of thrombin to TM induces a negative feedback loop that stops the coagulation.	bind
31203	2	7576	7	NULL	NULL	0	NULL	statement 1	NULL		induces	NULL				negative feedback loop	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_10_1292_s_22	8857927	3  Thus, binding of thrombin to TM induces a negative feedback loop that stops the coagulation.	bind
31204	3	7576	7	NULL	NULL	0	NULL	statement 2	NULL		stops	NULL				coagulation	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_10_1292_s_22	8857927	3  Thus, binding of thrombin to TM induces a negative feedback loop that stops the coagulation.	bind
28680	1	7578	5	13	NULL	NULL	NULL	LDL	GP	very early form of oxidized 	bind					CD14	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1213_s_27	15718493	3 - 5   We demonstrated recently that a very early form of oxidized LDL, minimally modified LDL (mmLDL), binds to the LPS receptor CD14 and stimulates macrophage spreading and actin polymerization.	bind
28681	2	7578	5	13	NULL	NULL	NULL	CD14	GP		is a type of					LPS receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1213_s_27	15718493	3 - 5   We demonstrated recently that a very early form of oxidized LDL, minimally modified LDL (mmLDL), binds to the LPS receptor CD14 and stimulates macrophage spreading and actin polymerization.	bind
28682	3	7578	5	13	NULL	NULL	NULL	mmLDL	GP		is					minimally modified LDL	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1213_s_27	15718493	3 - 5   We demonstrated recently that a very early form of oxidized LDL, minimally modified LDL (mmLDL), binds to the LPS receptor CD14 and stimulates macrophage spreading and actin polymerization.	bind
28683	4	7578	5	13	NULL	NULL	NULL	mmLDL	GP		bind					CD14	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1213_s_27	15718493	3 - 5   We demonstrated recently that a very early form of oxidized LDL, minimally modified LDL (mmLDL), binds to the LPS receptor CD14 and stimulates macrophage spreading and actin polymerization.	bind
28684	5	7578	5	13	NULL	NULL	NULL	statement 1	Process		stimulates					macrophage	Cell	spreading of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1213_s_27	15718493	3 - 5   We demonstrated recently that a very early form of oxidized LDL, minimally modified LDL (mmLDL), binds to the LPS receptor CD14 and stimulates macrophage spreading and actin polymerization.	bind
28685	6	7578	5	13	NULL	NULL	NULL	statement 4	Process		stimulates					macrophage	Cell	spreading of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1213_s_27	15718493	3 - 5   We demonstrated recently that a very early form of oxidized LDL, minimally modified LDL (mmLDL), binds to the LPS receptor CD14 and stimulates macrophage spreading and actin polymerization.	bind
28686	7	7578	5	13	NULL	NULL	NULL	statement 1	Process		stimulates					actin	GP	polymerization of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1213_s_27	15718493	3 - 5   We demonstrated recently that a very early form of oxidized LDL, minimally modified LDL (mmLDL), binds to the LPS receptor CD14 and stimulates macrophage spreading and actin polymerization.	bind
28687	8	7578	5	13	NULL	NULL	NULL	statement 4	Process		stimulates					actin	GP	polymerization of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1213_s_27	15718493	3 - 5   We demonstrated recently that a very early form of oxidized LDL, minimally modified LDL (mmLDL), binds to the LPS receptor CD14 and stimulates macrophage spreading and actin polymerization.	bind
31205	1	7578	7	10	NULL	0	NULL	LDL		early form of oxidized	binds to					CD14					NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1213_s_27	15718493	3 - 5   We demonstrated recently that a very early form of oxidized LDL, minimally modified LDL (mmLDL), binds to the LPS receptor CD14 and stimulates macrophage spreading and actin polymerization.	bind
31206	2	7578	7	NULL	NULL	0	NULL	mmLDL	NULL		binds to	NULL				CD14	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1213_s_27	15718493	3 - 5   We demonstrated recently that a very early form of oxidized LDL, minimally modified LDL (mmLDL), binds to the LPS receptor CD14 and stimulates macrophage spreading and actin polymerization.	bind
31207	3	7578	7	10	NULL	0	NULL	statement 1			stimulate					macrophage		spreading of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1213_s_27	15718493	3 - 5   We demonstrated recently that a very early form of oxidized LDL, minimally modified LDL (mmLDL), binds to the LPS receptor CD14 and stimulates macrophage spreading and actin polymerization.	bind
31208	4	7578	7	10	NULL	0	NULL	statement 2			stimulate					macrophage		spreading of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1213_s_27	15718493	3 - 5   We demonstrated recently that a very early form of oxidized LDL, minimally modified LDL (mmLDL), binds to the LPS receptor CD14 and stimulates macrophage spreading and actin polymerization.	bind
31209	5	7578	7	NULL	NULL	0	NULL	statement 1	NULL		stimulate	NULL				actin	NULL	polymerization of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1213_s_27	15718493	3 - 5   We demonstrated recently that a very early form of oxidized LDL, minimally modified LDL (mmLDL), binds to the LPS receptor CD14 and stimulates macrophage spreading and actin polymerization.	bind
31210	6	7578	7	NULL	NULL	0	NULL	statement 2	NULL		stimulate	NULL				actin	NULL	polymerization of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1213_s_27	15718493	3 - 5   We demonstrated recently that a very early form of oxidized LDL, minimally modified LDL (mmLDL), binds to the LPS receptor CD14 and stimulates macrophage spreading and actin polymerization.	bind
31211	7	7578	7	NULL	NULL	0	NULL	CD14	NULL		is a type of	NULL				LPS receptor	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1213_s_27	15718493	3 - 5   We demonstrated recently that a very early form of oxidized LDL, minimally modified LDL (mmLDL), binds to the LPS receptor CD14 and stimulates macrophage spreading and actin polymerization.	bind
31212	8	7578	7	NULL	NULL	0	NULL	mmLDL	NULL		is	NULL				minimally modified LDL	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1213_s_27	15718493	3 - 5   We demonstrated recently that a very early form of oxidized LDL, minimally modified LDL (mmLDL), binds to the LPS receptor CD14 and stimulates macrophage spreading and actin polymerization.	bind
28688	1	7579	5	13	NULL	NULL	NULL	TBPS	Chemical		bind					GABAA receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainres_813_2_343_s_165	9838187	3 -hydroxy steroids are known to inhibit [35]TBPS binding to GABAA receptors with IC50 values in the nanomolar range [ 15,  17], therefore in the present study we wanted to verify that steroid-inhibition of [3]GHB binding was not mediated by GABAA receptors.	bind
28689	2	7579	5	13	NULL	NULL	NULL	3 -hydroxy steroids	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_brainres_813_2_343_s_165	9838187	3 -hydroxy steroids are known to inhibit [35]TBPS binding to GABAA receptors with IC50 values in the nanomolar range [ 15,  17], therefore in the present study we wanted to verify that steroid-inhibition of [3]GHB binding was not mediated by GABAA receptors.	bind
31213	1	7579	7	10	NULL	0	NULL	TBPS			bind					GABAA receptors					NULL		NULL	NULL	NULL	NULL	gw60_brainres_813_2_343_s_165	9838187	3 -hydroxy steroids are known to inhibit [35]TBPS binding to GABAA receptors with IC50 values in the nanomolar range [ 15,  17], therefore in the present study we wanted to verify that steroid-inhibition of [3]GHB binding was not mediated by GABAA receptors.	bind
31214	2	7579	7	NULL	NULL	0	NULL	3 -hydroxy steroids	NULL		inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_brainres_813_2_343_s_165	9838187	3 -hydroxy steroids are known to inhibit [35]TBPS binding to GABAA receptors with IC50 values in the nanomolar range [ 15,  17], therefore in the present study we wanted to verify that steroid-inhibition of [3]GHB binding was not mediated by GABAA receptors.	bind
28699	1	7580	5	13	NULL	NULL	NULL	angiotensin II	GP		elicits					smooth muscle	OrganismPart	contractions of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_76_2_310_s_144	7834843	3 21  A number of recent reports have suggested that contractions of smooth muscle elicited by agonists such as angiotensin II and noradrenaline, which stimulate G protein - linked receptors, are mediated in part by as-yet-unidentified PTKs. 5  6  It is also the case that orthovanadate, which blocks tyrosine phosphatases, induces smooth muscle contraction in parallel with tyrosine phosphorylation of as-yet-unidentified cellular proteins 20  and that several growth factors that are known to bind to receptor tyrosine kinases cause tension development.	bind
28700	2	7580	5	13	NULL	NULL	NULL	noradrenaline	Chemical		elicits					smooth muscle	OrganismPart	contractions of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_76_2_310_s_144	7834843	3 21  A number of recent reports have suggested that contractions of smooth muscle elicited by agonists such as angiotensin II and noradrenaline, which stimulate G protein - linked receptors, are mediated in part by as-yet-unidentified PTKs. 5  6  It is also the case that orthovanadate, which blocks tyrosine phosphatases, induces smooth muscle contraction in parallel with tyrosine phosphorylation of as-yet-unidentified cellular proteins 20  and that several growth factors that are known to bind to receptor tyrosine kinases cause tension development.	bind
28701	3	7580	5	13	NULL	NULL	NULL	angiotensin II	GP		is a type of					agonist	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_76_2_310_s_144	7834843	3 21  A number of recent reports have suggested that contractions of smooth muscle elicited by agonists such as angiotensin II and noradrenaline, which stimulate G protein - linked receptors, are mediated in part by as-yet-unidentified PTKs. 5  6  It is also the case that orthovanadate, which blocks tyrosine phosphatases, induces smooth muscle contraction in parallel with tyrosine phosphorylation of as-yet-unidentified cellular proteins 20  and that several growth factors that are known to bind to receptor tyrosine kinases cause tension development.	bind
28702	4	7580	5	13	NULL	NULL	NULL	noradrenaline	Chemical		is a type of					agonist	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_76_2_310_s_144	7834843	3 21  A number of recent reports have suggested that contractions of smooth muscle elicited by agonists such as angiotensin II and noradrenaline, which stimulate G protein - linked receptors, are mediated in part by as-yet-unidentified PTKs. 5  6  It is also the case that orthovanadate, which blocks tyrosine phosphatases, induces smooth muscle contraction in parallel with tyrosine phosphorylation of as-yet-unidentified cellular proteins 20  and that several growth factors that are known to bind to receptor tyrosine kinases cause tension development.	bind
28703	5	7580	5	13	NULL	NULL	NULL	angiotensin II	GP		stimulates					G protein - linked receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_76_2_310_s_144	7834843	3 21  A number of recent reports have suggested that contractions of smooth muscle elicited by agonists such as angiotensin II and noradrenaline, which stimulate G protein - linked receptors, are mediated in part by as-yet-unidentified PTKs. 5  6  It is also the case that orthovanadate, which blocks tyrosine phosphatases, induces smooth muscle contraction in parallel with tyrosine phosphorylation of as-yet-unidentified cellular proteins 20  and that several growth factors that are known to bind to receptor tyrosine kinases cause tension development.	bind
28704	6	7580	5	13	NULL	NULL	NULL	noradrenaline	Chemical		stimulates					G protein - linked receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_76_2_310_s_144	7834843	3 21  A number of recent reports have suggested that contractions of smooth muscle elicited by agonists such as angiotensin II and noradrenaline, which stimulate G protein - linked receptors, are mediated in part by as-yet-unidentified PTKs. 5  6  It is also the case that orthovanadate, which blocks tyrosine phosphatases, induces smooth muscle contraction in parallel with tyrosine phosphorylation of as-yet-unidentified cellular proteins 20  and that several growth factors that are known to bind to receptor tyrosine kinases cause tension development.	bind
28705	7	7580	5	13	NULL	NULL	NULL	PTKs	GP	unidentified	mediate		partly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_76_2_310_s_144	7834843	3 21  A number of recent reports have suggested that contractions of smooth muscle elicited by agonists such as angiotensin II and noradrenaline, which stimulate G protein - linked receptors, are mediated in part by as-yet-unidentified PTKs. 5  6  It is also the case that orthovanadate, which blocks tyrosine phosphatases, induces smooth muscle contraction in parallel with tyrosine phosphorylation of as-yet-unidentified cellular proteins 20  and that several growth factors that are known to bind to receptor tyrosine kinases cause tension development.	bind
28706	8	7580	5	13	NULL	NULL	NULL	PTKs	GP	unidentified	mediate		partly			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_76_2_310_s_144	7834843	3 21  A number of recent reports have suggested that contractions of smooth muscle elicited by agonists such as angiotensin II and noradrenaline, which stimulate G protein - linked receptors, are mediated in part by as-yet-unidentified PTKs. 5  6  It is also the case that orthovanadate, which blocks tyrosine phosphatases, induces smooth muscle contraction in parallel with tyrosine phosphorylation of as-yet-unidentified cellular proteins 20  and that several growth factors that are known to bind to receptor tyrosine kinases cause tension development.	bind
28707	9	7580	5	13	NULL	NULL	NULL	orthovanadate	Chemical		blocks					tyrosine phosphatases	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_76_2_310_s_144	7834843	3 21  A number of recent reports have suggested that contractions of smooth muscle elicited by agonists such as angiotensin II and noradrenaline, which stimulate G protein - linked receptors, are mediated in part by as-yet-unidentified PTKs. 5  6  It is also the case that orthovanadate, which blocks tyrosine phosphatases, induces smooth muscle contraction in parallel with tyrosine phosphorylation of as-yet-unidentified cellular proteins 20  and that several growth factors that are known to bind to receptor tyrosine kinases cause tension development.	bind
28708	10	7580	5	13	NULL	NULL	NULL	orthovanadate	Chemical		induces					smooth muscle	OrganismPart	contractions of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_76_2_310_s_144	7834843	3 21  A number of recent reports have suggested that contractions of smooth muscle elicited by agonists such as angiotensin II and noradrenaline, which stimulate G protein - linked receptors, are mediated in part by as-yet-unidentified PTKs. 5  6  It is also the case that orthovanadate, which blocks tyrosine phosphatases, induces smooth muscle contraction in parallel with tyrosine phosphorylation of as-yet-unidentified cellular proteins 20  and that several growth factors that are known to bind to receptor tyrosine kinases cause tension development.	bind
28709	11	7580	5	13	NULL	NULL	NULL	orthovanadate	Chemical		phosphorylates					cellular proteins	GP	unidentified	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_76_2_310_s_144	7834843	3 21  A number of recent reports have suggested that contractions of smooth muscle elicited by agonists such as angiotensin II and noradrenaline, which stimulate G protein - linked receptors, are mediated in part by as-yet-unidentified PTKs. 5  6  It is also the case that orthovanadate, which blocks tyrosine phosphatases, induces smooth muscle contraction in parallel with tyrosine phosphorylation of as-yet-unidentified cellular proteins 20  and that several growth factors that are known to bind to receptor tyrosine kinases cause tension development.	bind
28710	12	7580	5	13	NULL	NULL	NULL	growth factors	GP		bind					receptor tyrosine kinases	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_76_2_310_s_144	7834843	3 21  A number of recent reports have suggested that contractions of smooth muscle elicited by agonists such as angiotensin II and noradrenaline, which stimulate G protein - linked receptors, are mediated in part by as-yet-unidentified PTKs. 5  6  It is also the case that orthovanadate, which blocks tyrosine phosphatases, induces smooth muscle contraction in parallel with tyrosine phosphorylation of as-yet-unidentified cellular proteins 20  and that several growth factors that are known to bind to receptor tyrosine kinases cause tension development.	bind
28711	13	7580	5	13	NULL	NULL	NULL	statement 12	Process		causes					tension development	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_76_2_310_s_144	7834843	3 21  A number of recent reports have suggested that contractions of smooth muscle elicited by agonists such as angiotensin II and noradrenaline, which stimulate G protein - linked receptors, are mediated in part by as-yet-unidentified PTKs. 5  6  It is also the case that orthovanadate, which blocks tyrosine phosphatases, induces smooth muscle contraction in parallel with tyrosine phosphorylation of as-yet-unidentified cellular proteins 20  and that several growth factors that are known to bind to receptor tyrosine kinases cause tension development.	bind
54561	14	7580	5	13	NULL	NULL	NULL	statement 10	Process		occurs in parallel with					statement 11	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_76_2_310_s_144	7834843	3 21  A number of recent reports have suggested that contractions of smooth muscle elicited by agonists such as angiotensin II and noradrenaline, which stimulate G protein - linked receptors, are mediated in part by as-yet-unidentified PTKs. 5  6  It is also the case that orthovanadate, which blocks tyrosine phosphatases, induces smooth muscle contraction in parallel with tyrosine phosphorylation of as-yet-unidentified cellular proteins 20  and that several growth factors that are known to bind to receptor tyrosine kinases cause tension development.	bind
31217	1	7580	7	NULL	NULL	0	NULL	angiotensin II	NULL		elicits	NULL				smooth muscle contractions	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_76_2_310_s_144	7834843	3 21  A number of recent reports have suggested that contractions of smooth muscle elicited by agonists such as angiotensin II and noradrenaline, which stimulate G protein - linked receptors, are mediated in part by as-yet-unidentified PTKs. 5  6  It is also the case that orthovanadate, which blocks tyrosine phosphatases, induces smooth muscle contraction in parallel with tyrosine phosphorylation of as-yet-unidentified cellular proteins 20  and that several growth factors that are known to bind to receptor tyrosine kinases cause tension development.	bind
31218	2	7580	7	NULL	NULL	0	NULL	noradrenaline	NULL		elicits	NULL				smooth muscle contractions	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_76_2_310_s_144	7834843	3 21  A number of recent reports have suggested that contractions of smooth muscle elicited by agonists such as angiotensin II and noradrenaline, which stimulate G protein - linked receptors, are mediated in part by as-yet-unidentified PTKs. 5  6  It is also the case that orthovanadate, which blocks tyrosine phosphatases, induces smooth muscle contraction in parallel with tyrosine phosphorylation of as-yet-unidentified cellular proteins 20  and that several growth factors that are known to bind to receptor tyrosine kinases cause tension development.	bind
31219	3	7580	7	NULL	NULL	0	NULL	angiotensin II 	NULL		stimulate	NULL				G protein - linked receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_76_2_310_s_144	7834843	3 21  A number of recent reports have suggested that contractions of smooth muscle elicited by agonists such as angiotensin II and noradrenaline, which stimulate G protein - linked receptors, are mediated in part by as-yet-unidentified PTKs. 5  6  It is also the case that orthovanadate, which blocks tyrosine phosphatases, induces smooth muscle contraction in parallel with tyrosine phosphorylation of as-yet-unidentified cellular proteins 20  and that several growth factors that are known to bind to receptor tyrosine kinases cause tension development.	bind
31220	4	7580	7	NULL	NULL	0	NULL	noradrenaline	NULL		stimulate	NULL				G protein - linked receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_76_2_310_s_144	7834843	3 21  A number of recent reports have suggested that contractions of smooth muscle elicited by agonists such as angiotensin II and noradrenaline, which stimulate G protein - linked receptors, are mediated in part by as-yet-unidentified PTKs. 5  6  It is also the case that orthovanadate, which blocks tyrosine phosphatases, induces smooth muscle contraction in parallel with tyrosine phosphorylation of as-yet-unidentified cellular proteins 20  and that several growth factors that are known to bind to receptor tyrosine kinases cause tension development.	bind
31221	5	7580	7	NULL	NULL	0	NULL	unidentified PTKs	NULL		mediates	NULL	partly			statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_76_2_310_s_144	7834843	3 21  A number of recent reports have suggested that contractions of smooth muscle elicited by agonists such as angiotensin II and noradrenaline, which stimulate G protein - linked receptors, are mediated in part by as-yet-unidentified PTKs. 5  6  It is also the case that orthovanadate, which blocks tyrosine phosphatases, induces smooth muscle contraction in parallel with tyrosine phosphorylation of as-yet-unidentified cellular proteins 20  and that several growth factors that are known to bind to receptor tyrosine kinases cause tension development.	bind
31222	6	7580	7	NULL	NULL	0	NULL	unidentified PTKs	NULL		mediates	NULL	partly			statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_76_2_310_s_144	7834843	3 21  A number of recent reports have suggested that contractions of smooth muscle elicited by agonists such as angiotensin II and noradrenaline, which stimulate G protein - linked receptors, are mediated in part by as-yet-unidentified PTKs. 5  6  It is also the case that orthovanadate, which blocks tyrosine phosphatases, induces smooth muscle contraction in parallel with tyrosine phosphorylation of as-yet-unidentified cellular proteins 20  and that several growth factors that are known to bind to receptor tyrosine kinases cause tension development.	bind
31223	7	7580	7	NULL	NULL	0	NULL	orthovanadate	NULL		blocks	NULL				tyrosine phosphatases	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_76_2_310_s_144	7834843	3 21  A number of recent reports have suggested that contractions of smooth muscle elicited by agonists such as angiotensin II and noradrenaline, which stimulate G protein - linked receptors, are mediated in part by as-yet-unidentified PTKs. 5  6  It is also the case that orthovanadate, which blocks tyrosine phosphatases, induces smooth muscle contraction in parallel with tyrosine phosphorylation of as-yet-unidentified cellular proteins 20  and that several growth factors that are known to bind to receptor tyrosine kinases cause tension development.	bind
31224	8	7580	7	NULL	NULL	0	NULL	statement 7	NULL		induces	NULL				smooth muscle contraction	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_76_2_310_s_144	7834843	3 21  A number of recent reports have suggested that contractions of smooth muscle elicited by agonists such as angiotensin II and noradrenaline, which stimulate G protein - linked receptors, are mediated in part by as-yet-unidentified PTKs. 5  6  It is also the case that orthovanadate, which blocks tyrosine phosphatases, induces smooth muscle contraction in parallel with tyrosine phosphorylation of as-yet-unidentified cellular proteins 20  and that several growth factors that are known to bind to receptor tyrosine kinases cause tension development.	bind
31225	9	7580	7	NULL	NULL	0	NULL	orthovanadate	NULL		phosphorylates	NULL				unidentified cellular proteins	NULL		tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_76_2_310_s_144	7834843	3 21  A number of recent reports have suggested that contractions of smooth muscle elicited by agonists such as angiotensin II and noradrenaline, which stimulate G protein - linked receptors, are mediated in part by as-yet-unidentified PTKs. 5  6  It is also the case that orthovanadate, which blocks tyrosine phosphatases, induces smooth muscle contraction in parallel with tyrosine phosphorylation of as-yet-unidentified cellular proteins 20  and that several growth factors that are known to bind to receptor tyrosine kinases cause tension development.	bind
31226	10	7580	7	NULL	NULL	0	NULL	statement 8	NULL		occurs in parallel with	NULL				statement 9	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_76_2_310_s_144	7834843	3 21  A number of recent reports have suggested that contractions of smooth muscle elicited by agonists such as angiotensin II and noradrenaline, which stimulate G protein - linked receptors, are mediated in part by as-yet-unidentified PTKs. 5  6  It is also the case that orthovanadate, which blocks tyrosine phosphatases, induces smooth muscle contraction in parallel with tyrosine phosphorylation of as-yet-unidentified cellular proteins 20  and that several growth factors that are known to bind to receptor tyrosine kinases cause tension development.	bind
31227	11	7580	7	NULL	NULL	0	NULL	growth factors	NULL		bind	NULL				 receptor tyrosine kinases	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_76_2_310_s_144	7834843	3 21  A number of recent reports have suggested that contractions of smooth muscle elicited by agonists such as angiotensin II and noradrenaline, which stimulate G protein - linked receptors, are mediated in part by as-yet-unidentified PTKs. 5  6  It is also the case that orthovanadate, which blocks tyrosine phosphatases, induces smooth muscle contraction in parallel with tyrosine phosphorylation of as-yet-unidentified cellular proteins 20  and that several growth factors that are known to bind to receptor tyrosine kinases cause tension development.	bind
31228	12	7580	7	NULL	NULL	0	NULL	statement 11	NULL		cause	NULL				tension development	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_76_2_310_s_144	7834843	3 21  A number of recent reports have suggested that contractions of smooth muscle elicited by agonists such as angiotensin II and noradrenaline, which stimulate G protein - linked receptors, are mediated in part by as-yet-unidentified PTKs. 5  6  It is also the case that orthovanadate, which blocks tyrosine phosphatases, induces smooth muscle contraction in parallel with tyrosine phosphorylation of as-yet-unidentified cellular proteins 20  and that several growth factors that are known to bind to receptor tyrosine kinases cause tension development.	bind
31234	13	7580	7	NULL	NULL	0	NULL	angiotensin II	NULL		is a type of	NULL				agonist	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_76_2_310_s_144	7834843	3 21  A number of recent reports have suggested that contractions of smooth muscle elicited by agonists such as angiotensin II and noradrenaline, which stimulate G protein - linked receptors, are mediated in part by as-yet-unidentified PTKs. 5  6  It is also the case that orthovanadate, which blocks tyrosine phosphatases, induces smooth muscle contraction in parallel with tyrosine phosphorylation of as-yet-unidentified cellular proteins 20  and that several growth factors that are known to bind to receptor tyrosine kinases cause tension development.	bind
31235	14	7580	7	NULL	NULL	0	NULL	noradrenaline	NULL		is a type of	NULL				agonist	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_76_2_310_s_144	7834843	3 21  A number of recent reports have suggested that contractions of smooth muscle elicited by agonists such as angiotensin II and noradrenaline, which stimulate G protein - linked receptors, are mediated in part by as-yet-unidentified PTKs. 5  6  It is also the case that orthovanadate, which blocks tyrosine phosphatases, induces smooth muscle contraction in parallel with tyrosine phosphorylation of as-yet-unidentified cellular proteins 20  and that several growth factors that are known to bind to receptor tyrosine kinases cause tension development.	bind
28712	1	7581	5	13	NULL	NULL	NULL	fibrinogen	GP		bind					GPIIb-IIIa	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_5_621_s_20	8963718	3 4 5  6  Binding of fibrinogen to GPIIb-IIIa is mediated through amino acid sequences present in regions of the alpha and gamma chains of the fibrinogen macromolecule.	bind
28713	2	7581	5	13	NULL	NULL	NULL	statement 1	Process		is mediated through					fibrinogen macromolecule	GP		alpha chains amino acid		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_5_621_s_20	8963718	3 4 5  6  Binding of fibrinogen to GPIIb-IIIa is mediated through amino acid sequences present in regions of the alpha and gamma chains of the fibrinogen macromolecule.	bind
28714	3	7581	5	13	NULL	NULL	NULL	statement 1	Process		is mediated through					fibrinogen macromolecule	GP		gamma chain amino acid		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_5_621_s_20	8963718	3 4 5  6  Binding of fibrinogen to GPIIb-IIIa is mediated through amino acid sequences present in regions of the alpha and gamma chains of the fibrinogen macromolecule.	bind
31229	1	7581	7	10	NULL	0	NULL	fibrinogen	NULL		bind	NULL				GPIIb-IIIa	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_5_621_s_20	8963718	3 4 5  6  Binding of fibrinogen to GPIIb-IIIa is mediated through amino acid sequences present in regions of the alpha and gamma chains of the fibrinogen macromolecule.	bind
31230	2	7581	7	10	NULL	0	NULL	statement 1	NULL		is mediated through	NULL				fibrinogen macromolecule	NULL		alpha chains amino acid		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_5_621_s_20	8963718	3 4 5  6  Binding of fibrinogen to GPIIb-IIIa is mediated through amino acid sequences present in regions of the alpha and gamma chains of the fibrinogen macromolecule.	bind
46657	3	7581	7	10	NULL	0	NULL	statement 1	NULL		is mediated through	NULL				fibrinogen macromolecule	NULL		gamma chain amino acid		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_5_621_s_20	8963718	3 4 5  6  Binding of fibrinogen to GPIIb-IIIa is mediated through amino acid sequences present in regions of the alpha and gamma chains of the fibrinogen macromolecule.	bind
28690	1	7582	5	13	NULL	NULL	NULL	Ang II	GP		bind					AT1s	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_8_710_s_17	11029408	3 4 5  Binding of Ang II to AT1s activates several signaling pathways implicated in regulating cellular growth.	bind
28715	2	7582	5	13	NULL	NULL	NULL	statement 1	Process		activates					signaling pathways	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_8_710_s_17	11029408	3 4 5  Binding of Ang II to AT1s activates several signaling pathways implicated in regulating cellular growth.	bind
46658	3	7582	5	13	NULL	NULL	NULL	statement 2	Process		implicated in					cellular growth	Process	regulation of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_8_710_s_17	11029408	3 4 5  Binding of Ang II to AT1s activates several signaling pathways implicated in regulating cellular growth.	bind
31231	1	7582	7	NULL	NULL	0	NULL	Ang II	NULL		bind	NULL				AT1s	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_8_710_s_17	11029408	3 4 5  Binding of Ang II to AT1s activates several signaling pathways implicated in regulating cellular growth.	bind
31232	2	7582	7	NULL	NULL	0	NULL	statement 1	NULL		activates	NULL				signaling pathways	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_8_710_s_17	11029408	3 4 5  Binding of Ang II to AT1s activates several signaling pathways implicated in regulating cellular growth.	bind
31233	3	7582	7	NULL	NULL	0	NULL	statement 2	NULL		implicated in	NULL				cellular growth	NULL	regulation of			NULL		0	NULL	NULL	NULL	gw60_circulationres_87_8_710_s_17	11029408	3 4 5  Binding of Ang II to AT1s activates several signaling pathways implicated in regulating cellular growth.	bind
28716	1	7584	5	13	NULL	NULL	NULL	c7E3	GP		is a type of					monoclonal IgG Fab antibody fragment	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_94_5_906_s_21	8790024	3 4 5 6  The currently available parenteral GP IIb/IIa receptor antagonist is a monoclonal IgG Fab antibody fragment (c7E3, abciximab [ReoPro] Centocor, Inc) that binds the GP IIb/IIa receptor with high affinity, resulting in a long biological half-life.	bind
28717	2	7584	5	13	NULL	NULL	NULL	c7E3	GP		is antagonist of					GP IIb/IIa receptor	GP	parenteral			NULL		NULL	NULL	NULL	NULL	gw60_circulation_94_5_906_s_21	8790024	3 4 5 6  The currently available parenteral GP IIb/IIa receptor antagonist is a monoclonal IgG Fab antibody fragment (c7E3, abciximab [ReoPro] Centocor, Inc) that binds the GP IIb/IIa receptor with high affinity, resulting in a long biological half-life.	bind
28718	3	7584	5	13	NULL	NULL	NULL	c7E3	GP		bind		high affinity			GP IIb/IIa receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_94_5_906_s_21	8790024	3 4 5 6  The currently available parenteral GP IIb/IIa receptor antagonist is a monoclonal IgG Fab antibody fragment (c7E3, abciximab [ReoPro] Centocor, Inc) that binds the GP IIb/IIa receptor with high affinity, resulting in a long biological half-life.	bind
28719	4	7584	5	13	NULL	NULL	NULL	statement 3	Process		results in					biological half-life	Process	long			NULL		NULL	NULL	NULL	NULL	gw60_circulation_94_5_906_s_21	8790024	3 4 5 6  The currently available parenteral GP IIb/IIa receptor antagonist is a monoclonal IgG Fab antibody fragment (c7E3, abciximab [ReoPro] Centocor, Inc) that binds the GP IIb/IIa receptor with high affinity, resulting in a long biological half-life.	bind
31236	1	7584	7	NULL	NULL	0	NULL	c7E3	NULL		binds	NULL	high affinity			GP IIb/IIa receptor	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_94_5_906_s_21	8790024	3 4 5 6  The currently available parenteral GP IIb/IIa receptor antagonist is a monoclonal IgG Fab antibody fragment (c7E3, abciximab [ReoPro] Centocor, Inc) that binds the GP IIb/IIa receptor with high affinity, resulting in a long biological half-life.	bind
31237	2	7584	7	NULL	NULL	0	NULL	c7E3	NULL		is a type of	NULL				monoclonal IgG Fab antibody fragment	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_94_5_906_s_21	8790024	3 4 5 6  The currently available parenteral GP IIb/IIa receptor antagonist is a monoclonal IgG Fab antibody fragment (c7E3, abciximab [ReoPro] Centocor, Inc) that binds the GP IIb/IIa receptor with high affinity, resulting in a long biological half-life.	bind
31238	4	7584	7	10	NULL	0	NULL	statement 1			results in					biological half-life		 long			NULL		NULL	NULL	NULL	NULL	gw60_circulation_94_5_906_s_21	8790024	3 4 5 6  The currently available parenteral GP IIb/IIa receptor antagonist is a monoclonal IgG Fab antibody fragment (c7E3, abciximab [ReoPro] Centocor, Inc) that binds the GP IIb/IIa receptor with high affinity, resulting in a long biological half-life.	bind
46724	3	7584	7	10	NULL	0	NULL	c7E3	NULL		is antagonist of	NULL				 GP IIb/IIa receptor 	NULL	parenteral			NULL		NULL	NULL	NULL	NULL	gw60_circulation_94_5_906_s_21	8790024	3 4 5 6  The currently available parenteral GP IIb/IIa receptor antagonist is a monoclonal IgG Fab antibody fragment (c7E3, abciximab [ReoPro] Centocor, Inc) that binds the GP IIb/IIa receptor with high affinity, resulting in a long biological half-life.	bind
28720	1	7585	5	13	NULL	NULL	NULL				bind			L2 domain		E1a kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_10_6361_s_34	9045657	3 4 The L2 domain binds the E1a kinase ( 30) and the E1b phosphatase ( 31).	bind
28721	2	7585	5	13	NULL	NULL	NULL				bind			L2 domain		E1b phosphatase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_10_6361_s_34	9045657	3 4 The L2 domain binds the E1a kinase ( 30) and the E1b phosphatase ( 31).	bind
31239	1	7585	7	NULL	NULL	0	NULL		NULL		binds	NULL		L2 domain		E1a kinase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_10_6361_s_34	9045657	3 4 The L2 domain binds the E1a kinase ( 30) and the E1b phosphatase ( 31).	bind
31240	2	7585	7	NULL	NULL	0	NULL		NULL		binds	NULL		L2 domain		E1b phosphatase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_10_6361_s_34	9045657	3 4 The L2 domain binds the E1a kinase ( 30) and the E1b phosphatase ( 31).	bind
28722	1	7586	5	13	NULL	NULL	NULL	apoA-I	GP		bind					phospholipids	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1426_s_22	15845909	3 4F is an apoA-I mimetic peptide that binds phospholipids similar to apoA-I.	bind
28723	2	7586	5	13	NULL	NULL	NULL	4F	GP		is a type of					apoA-I mimetic peptide	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1426_s_22	15845909	3 4F is an apoA-I mimetic peptide that binds phospholipids similar to apoA-I.	bind
28724	3	7586	5	13	NULL	NULL	NULL	4F	GP		bind					phospholipids	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1426_s_22	15845909	3 4F is an apoA-I mimetic peptide that binds phospholipids similar to apoA-I.	bind
31241	1	7586	7	NULL	NULL	0	NULL	 4F	NULL		binds	NULL				phospholipids	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1426_s_22	15845909	3 4F is an apoA-I mimetic peptide that binds phospholipids similar to apoA-I.	bind
31242	2	7586	7	NULL	NULL	0	NULL	 4F	NULL		binds	NULL				apoA-I	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1426_s_22	15845909	3 4F is an apoA-I mimetic peptide that binds phospholipids similar to apoA-I.	bind
31243	3	7586	7	NULL	NULL	0	NULL	4F 	NULL		is a type of	NULL				apoA-I mimetic peptide	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1426_s_22	15845909	3 4F is an apoA-I mimetic peptide that binds phospholipids similar to apoA-I.	bind
28726	1	7587	5	13	NULL	NULL	NULL	apo B	GP		bind					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_2_505_s_66	7805256	3 8  The resulting amino acid substitution disrupts apo B binding to the LDL receptor, impairing LDL uptake.	bind
28727	2	7587	5	13	NULL	NULL	NULL	amino acid substitution	Process		disrupts					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_2_505_s_66	7805256	3 8  The resulting amino acid substitution disrupts apo B binding to the LDL receptor, impairing LDL uptake.	bind
28728	3	7587	5	13	NULL	NULL	NULL	statement 2	Process		impairs					LDL	GP	uptake of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_2_505_s_66	7805256	3 8  The resulting amino acid substitution disrupts apo B binding to the LDL receptor, impairing LDL uptake.	bind
31244	1	7587	7	NULL	NULL	0	NULL	apo B	NULL		bind	NULL				LDL receptor	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_2_505_s_66	7805256	3 8  The resulting amino acid substitution disrupts apo B binding to the LDL receptor, impairing LDL uptake.	bind
31245	2	7587	7	NULL	NULL	0	NULL	aminoacid substitution	NULL		disrupts	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_91_2_505_s_66	7805256	3 8  The resulting amino acid substitution disrupts apo B binding to the LDL receptor, impairing LDL uptake.	bind
31246	3	7587	7	NULL	NULL	0	NULL	statement 1	NULL		impairs	NULL				LDL	NULL	uptake of			NULL		0	NULL	NULL	NULL	gw60_circulation_91_2_505_s_66	7805256	3 8  The resulting amino acid substitution disrupts apo B binding to the LDL receptor, impairing LDL uptake.	bind
28729	1	7588	5	13	NULL	NULL	NULL	MutY	GP		bind		differentially	G116D		DNA	NucleicAcid	A/G-containing			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_39_24138_s_170	8798653	3 a result consistent with the differential binding of MutY(G116D) with A/G- and A/GO-containing DNA.	bind
28730	2	7588	5	13	NULL	NULL	NULL	MutY	GP		bind		differentially	G116D		DNA	NucleicAcid	A/GO-containing			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_39_24138_s_170	8798653	3 a result consistent with the differential binding of MutY(G116D) with A/G- and A/GO-containing DNA.	bind
31247	1	7588	7	10	NULL	0	NULL	MutY			bind		differentially	G116D		DNA		A/G containing			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_39_24138_s_170	8798653	3 a result consistent with the differential binding of MutY(G116D) with A/G- and A/GO-containing DNA.	bind
31248	2	7588	7	10	NULL	0	NULL	MutY			bind		differentially	G116D		DNA		A/GO-containing			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_39_24138_s_170	8798653	3 a result consistent with the differential binding of MutY(G116D) with A/G- and A/GO-containing DNA.	bind
29042	2	7589	5	13	NULL	NULL	NULL	MHC class I molecules	GP	viral	bind					MHC class I receptor	GP	viral			NULL		NULL	NULL	NULL	NULL	gw60_microbesinfect_2_5_521_s_215	10865197	3 A,B.  Cis-binding of the viral MHC class I molecules with its receptor may lead to inhibition of NK cell stimulatory cytokines, preventing NK cell recruitment and activation.	bind
29043	3	7589	5	13	NULL	NULL	NULL	statement 1	Process		prevents					NK cell	Cell	recruitment of			NULL		NULL	NULL	NULL	NULL	gw60_microbesinfect_2_5_521_s_215	10865197	3 A,B.  Cis-binding of the viral MHC class I molecules with its receptor may lead to inhibition of NK cell stimulatory cytokines, preventing NK cell recruitment and activation.	bind
29044	4	7589	5	13	NULL	NULL	NULL	statement 1	Process		prevents					NK cell	Cell	activation of			NULL		NULL	NULL	NULL	NULL	gw60_microbesinfect_2_5_521_s_215	10865197	3 A,B.  Cis-binding of the viral MHC class I molecules with its receptor may lead to inhibition of NK cell stimulatory cytokines, preventing NK cell recruitment and activation.	bind
46659	1	7589	5	13	NULL	NULL	NULL	NK cells	Cell		stimulate					cytokines	GP				NULL		NULL	NULL	NULL	NULL	gw60_microbesinfect_2_5_521_s_215	10865197	3 A,B.  Cis-binding of the viral MHC class I molecules with its receptor may lead to inhibition of NK cell stimulatory cytokines, preventing NK cell recruitment and activation.	bind
46660	5	7589	5	13	NULL	NULL	NULL	statement 2	Process		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_microbesinfect_2_5_521_s_215	10865197	3 A,B.  Cis-binding of the viral MHC class I molecules with its receptor may lead to inhibition of NK cell stimulatory cytokines, preventing NK cell recruitment and activation.	bind
31249	1	7589	7	10	NULL	0	NULL	MHC class I molecules 		viral	bind					MHC class I  receptor					NULL		NULL	NULL	NULL	NULL	gw60_microbesinfect_2_5_521_s_215	10865197	3 A,B.  Cis-binding of the viral MHC class I molecules with its receptor may lead to inhibition of NK cell stimulatory cytokines, preventing NK cell recruitment and activation.	bind
31250	2	7589	7	NULL	NULL	0	NULL	NK cells	NULL		stimulate	NULL				cytokines	NULL				NULL		0	NULL	NULL	NULL	gw60_microbesinfect_2_5_521_s_215	10865197	3 A,B.  Cis-binding of the viral MHC class I molecules with its receptor may lead to inhibition of NK cell stimulatory cytokines, preventing NK cell recruitment and activation.	bind
31251	3	7589	7	NULL	NULL	0	NULL	statement 1	NULL		inhibits	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_microbesinfect_2_5_521_s_215	10865197	3 A,B.  Cis-binding of the viral MHC class I molecules with its receptor may lead to inhibition of NK cell stimulatory cytokines, preventing NK cell recruitment and activation.	bind
31252	4	7589	7	NULL	NULL	0	NULL	statement 2	NULL		prevents	NULL				NK cell	NULL	recruitment of 			NULL		0	NULL	NULL	NULL	gw60_microbesinfect_2_5_521_s_215	10865197	3 A,B.  Cis-binding of the viral MHC class I molecules with its receptor may lead to inhibition of NK cell stimulatory cytokines, preventing NK cell recruitment and activation.	bind
31253	5	7589	7	NULL	NULL	0	NULL	statement 2	NULL		prevents	NULL				NK cell	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_microbesinfect_2_5_521_s_215	10865197	3 A,B.  Cis-binding of the viral MHC class I molecules with its receptor may lead to inhibition of NK cell stimulatory cytokines, preventing NK cell recruitment and activation.	bind
29045	1	7590	5	13	NULL	NULL	NULL	caspase-3	GP		is processed by					oligomeric Apaf-1-caspase-9 complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_12_8461_s_211	10722681	3 Active caspase-3 not bound to the Apaf-1 complex appears to represent caspase-3 that is processed by the oligomeric Apaf-1-caspase-9 complex and subsequently released from the complex ( 14,  23).	bind
29046	2	7590	5	13	NULL	NULL	NULL	caspase-3	GP	active	is not bound to					Apaf-1 complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_12_8461_s_211	10722681	3 Active caspase-3 not bound to the Apaf-1 complex appears to represent caspase-3 that is processed by the oligomeric Apaf-1-caspase-9 complex and subsequently released from the complex ( 14,  23).	bind
29047	3	7590	5	13	NULL	NULL	NULL	statement 2	Process		represents		appears to			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_12_8461_s_211	10722681	3 Active caspase-3 not bound to the Apaf-1 complex appears to represent caspase-3 that is processed by the oligomeric Apaf-1-caspase-9 complex and subsequently released from the complex ( 14,  23).	bind
29048	4	7590	5	13	NULL	NULL	NULL	caspase-3	GP		is released from		subsequently			oligomeric Apaf-1-caspase-9 complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_12_8461_s_211	10722681	3 Active caspase-3 not bound to the Apaf-1 complex appears to represent caspase-3 that is processed by the oligomeric Apaf-1-caspase-9 complex and subsequently released from the complex ( 14,  23).	bind
31254	1	7590	7	NULL	NULL	0	NULL	caspase-3	NULL	active	does not bind	NULL				Apaf-1 complex	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_12_8461_s_211	10722681	3 Active caspase-3 not bound to the Apaf-1 complex appears to represent caspase-3 that is processed by the oligomeric Apaf-1-caspase-9 complex and subsequently released from the complex ( 14,  23).	bind
31255	2	7590	7	NULL	NULL	0	NULL	oligomeric Apaf-1-caspase-9 complex	NULL		process	NULL				caspase-3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_12_8461_s_211	10722681	3 Active caspase-3 not bound to the Apaf-1 complex appears to represent caspase-3 that is processed by the oligomeric Apaf-1-caspase-9 complex and subsequently released from the complex ( 14,  23).	bind
31256	3	7590	7	NULL	NULL	0	NULL	statement 1	NULL		represent	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_12_8461_s_211	10722681	3 Active caspase-3 not bound to the Apaf-1 complex appears to represent caspase-3 that is processed by the oligomeric Apaf-1-caspase-9 complex and subsequently released from the complex ( 14,  23).	bind
31257	4	7590	7	10	NULL	0	NULL	caspase-3			is released from		subsequently			statement 2					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_12_8461_s_211	10722681	3 Active caspase-3 not bound to the Apaf-1 complex appears to represent caspase-3 that is processed by the oligomeric Apaf-1-caspase-9 complex and subsequently released from the complex ( 14,  23).	bind
29049	1	7591	5	13	NULL	NULL	NULL	FVII/VIIa	GP		is					plasma factor VII/VIIa	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_555_s_23	16385085	3 After vessel injury, plasma factor VII/VIIa (FVII/VIIa) binds to TF to form a TF:FVIIa complex, which activates FX and FIX, leading to thrombin generation, fibrin deposition, and platelet activation.	bind
29050	2	7591	5	13	NULL	NULL	NULL	FVII/VIIa	GP		bind					TF	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_555_s_23	16385085	3 After vessel injury, plasma factor VII/VIIa (FVII/VIIa) binds to TF to form a TF:FVIIa complex, which activates FX and FIX, leading to thrombin generation, fibrin deposition, and platelet activation.	bind
29051	3	7591	5	13	NULL	NULL	NULL	statement 2	GP		forms					TF:FVIIa complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_555_s_23	16385085	3 After vessel injury, plasma factor VII/VIIa (FVII/VIIa) binds to TF to form a TF:FVIIa complex, which activates FX and FIX, leading to thrombin generation, fibrin deposition, and platelet activation.	bind
29052	4	7591	5	13	NULL	NULL	NULL	statement 3	Process		occurs after					vessel injury	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_555_s_23	16385085	3 After vessel injury, plasma factor VII/VIIa (FVII/VIIa) binds to TF to form a TF:FVIIa complex, which activates FX and FIX, leading to thrombin generation, fibrin deposition, and platelet activation.	bind
29053	5	7591	5	13	NULL	NULL	NULL	statement 3	Process		activates					FX	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_555_s_23	16385085	3 After vessel injury, plasma factor VII/VIIa (FVII/VIIa) binds to TF to form a TF:FVIIa complex, which activates FX and FIX, leading to thrombin generation, fibrin deposition, and platelet activation.	bind
29054	6	7591	5	13	NULL	NULL	NULL	statement 3	Process		activates					FIX	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_555_s_23	16385085	3 After vessel injury, plasma factor VII/VIIa (FVII/VIIa) binds to TF to form a TF:FVIIa complex, which activates FX and FIX, leading to thrombin generation, fibrin deposition, and platelet activation.	bind
29055	7	7591	5	13	NULL	NULL	NULL	statement 5	Process		leads to					thrombin	GP	generation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_555_s_23	16385085	3 After vessel injury, plasma factor VII/VIIa (FVII/VIIa) binds to TF to form a TF:FVIIa complex, which activates FX and FIX, leading to thrombin generation, fibrin deposition, and platelet activation.	bind
29056	8	7591	5	13	NULL	NULL	NULL	statement 5	Process		leads to					fibrin	GP	deposition of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_555_s_23	16385085	3 After vessel injury, plasma factor VII/VIIa (FVII/VIIa) binds to TF to form a TF:FVIIa complex, which activates FX and FIX, leading to thrombin generation, fibrin deposition, and platelet activation.	bind
29057	9	7591	5	13	NULL	NULL	NULL	statement 5	Process		leads to					platelet	Cell	activation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_555_s_23	16385085	3 After vessel injury, plasma factor VII/VIIa (FVII/VIIa) binds to TF to form a TF:FVIIa complex, which activates FX and FIX, leading to thrombin generation, fibrin deposition, and platelet activation.	bind
29058	10	7591	5	13	NULL	NULL	NULL	statement 6	Process		leads to					thrombin	GP	generation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_555_s_23	16385085	3 After vessel injury, plasma factor VII/VIIa (FVII/VIIa) binds to TF to form a TF:FVIIa complex, which activates FX and FIX, leading to thrombin generation, fibrin deposition, and platelet activation.	bind
29059	11	7591	5	13	NULL	NULL	NULL	statement 6	Process		leads to					fibrin	GP	deposition of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_555_s_23	16385085	3 After vessel injury, plasma factor VII/VIIa (FVII/VIIa) binds to TF to form a TF:FVIIa complex, which activates FX and FIX, leading to thrombin generation, fibrin deposition, and platelet activation.	bind
29060	12	7591	5	13	NULL	NULL	NULL	statement 6	Process		leads to					platelet	Cell	activation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_555_s_23	16385085	3 After vessel injury, plasma factor VII/VIIa (FVII/VIIa) binds to TF to form a TF:FVIIa complex, which activates FX and FIX, leading to thrombin generation, fibrin deposition, and platelet activation.	bind
31258	1	7591	7	NULL	NULL	0	NULL	FVII/VIIa	NULL		bind	NULL				TF	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_555_s_23	16385085	3 After vessel injury, plasma factor VII/VIIa (FVII/VIIa) binds to TF to form a TF:FVIIa complex, which activates FX and FIX, leading to thrombin generation, fibrin deposition, and platelet activation.	bind
31259	2	7591	7	NULL	NULL	0	NULL	statement 1	NULL		forms	NULL				TF:FVIIa complex	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_555_s_23	16385085	3 After vessel injury, plasma factor VII/VIIa (FVII/VIIa) binds to TF to form a TF:FVIIa complex, which activates FX and FIX, leading to thrombin generation, fibrin deposition, and platelet activation.	bind
31260	3	7591	7	NULL	NULL	0	NULL	statement 1	NULL		occurs after	NULL				vessel injury	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_555_s_23	16385085	3 After vessel injury, plasma factor VII/VIIa (FVII/VIIa) binds to TF to form a TF:FVIIa complex, which activates FX and FIX, leading to thrombin generation, fibrin deposition, and platelet activation.	bind
31261	4	7591	7	NULL	NULL	0	NULL	statement 2	NULL		activates	NULL				FX	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_555_s_23	16385085	3 After vessel injury, plasma factor VII/VIIa (FVII/VIIa) binds to TF to form a TF:FVIIa complex, which activates FX and FIX, leading to thrombin generation, fibrin deposition, and platelet activation.	bind
31262	5	7591	7	NULL	NULL	0	NULL	statement 2	NULL		activates	NULL				FIX	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_555_s_23	16385085	3 After vessel injury, plasma factor VII/VIIa (FVII/VIIa) binds to TF to form a TF:FVIIa complex, which activates FX and FIX, leading to thrombin generation, fibrin deposition, and platelet activation.	bind
31263	6	7591	7	NULL	NULL	0	NULL	statement 4	NULL		leads to	NULL				thrombin	NULL	generation of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_555_s_23	16385085	3 After vessel injury, plasma factor VII/VIIa (FVII/VIIa) binds to TF to form a TF:FVIIa complex, which activates FX and FIX, leading to thrombin generation, fibrin deposition, and platelet activation.	bind
31264	7	7591	7	NULL	NULL	0	NULL	statement 5	NULL		leads to	NULL				thrombin	NULL	generation of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_555_s_23	16385085	3 After vessel injury, plasma factor VII/VIIa (FVII/VIIa) binds to TF to form a TF:FVIIa complex, which activates FX and FIX, leading to thrombin generation, fibrin deposition, and platelet activation.	bind
31265	8	7591	7	NULL	NULL	0	NULL	statement 4	NULL		leads to	NULL				fibrin	NULL	deposition of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_555_s_23	16385085	3 After vessel injury, plasma factor VII/VIIa (FVII/VIIa) binds to TF to form a TF:FVIIa complex, which activates FX and FIX, leading to thrombin generation, fibrin deposition, and platelet activation.	bind
31266	9	7591	7	NULL	NULL	0	NULL	statement 5	NULL		leads to	NULL				fibrin	NULL	deposition of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_555_s_23	16385085	3 After vessel injury, plasma factor VII/VIIa (FVII/VIIa) binds to TF to form a TF:FVIIa complex, which activates FX and FIX, leading to thrombin generation, fibrin deposition, and platelet activation.	bind
31267	10	7591	7	NULL	NULL	0	NULL	statement 4	NULL		leads to	NULL				platelet 	NULL	activation of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_555_s_23	16385085	3 After vessel injury, plasma factor VII/VIIa (FVII/VIIa) binds to TF to form a TF:FVIIa complex, which activates FX and FIX, leading to thrombin generation, fibrin deposition, and platelet activation.	bind
31268	11	7591	7	NULL	NULL	0	NULL	statement 5	NULL		leads to	NULL				platelet	NULL	activation of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_555_s_23	16385085	3 After vessel injury, plasma factor VII/VIIa (FVII/VIIa) binds to TF to form a TF:FVIIa complex, which activates FX and FIX, leading to thrombin generation, fibrin deposition, and platelet activation.	bind
31269	12	7591	7	NULL	NULL	0	NULL	FVII/VIIa	NULL		is	NULL				plasma factor VII/VIIa	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_3_555_s_23	16385085	3 After vessel injury, plasma factor VII/VIIa (FVII/VIIa) binds to TF to form a TF:FVIIa complex, which activates FX and FIX, leading to thrombin generation, fibrin deposition, and platelet activation.	bind
29061	1	7592	5	13	NULL	NULL	NULL	Raf	GP	baculoviral;; recombinant	bind					GST-14.3.3 fusion protein	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_40_23681_s_183	7559537	3 already bound to the baculoviral  recombinant Raf-1 polypeptide, such Raf preparations bind  in vitro  to a GST-14.3.3    fusion protein but not to GST alone ( Fig. 3,  upper panel,  lanes 1  and  2); preincubation of Raf with cleaved, purified  E. coli  recombinant 14.3.	bind
31270	1	7592	7	10	NULL	0	NULL	Raf-1 polypeptide	NULL	baculoviral;; recombinant	bind	NULL				GST-14.3.3 fusion protein	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_40_23681_s_183	7559537	3 already bound to the baculoviral  recombinant Raf-1 polypeptide, such Raf preparations bind  in vitro  to a GST-14.3.3    fusion protein but not to GST alone ( Fig. 3,  upper panel,  lanes 1  and  2); preincubation of Raf with cleaved, purified  E. coli  recombinant 14.3.	bind
29063	1	7593	5	13	NULL	NULL	NULL	procaspase-8	GP		bind					TRADD	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_40_39251_s_212	12882979	3 Alternatively, mechanisms to inhibit FADD and procaspase-8 binding to TRADD may exist, either by regulatory molecules physically blocking this association or preferentially enhancing the TRAF2 and RIP binding to TRADD.	bind
29064	3	7593	5	13	NULL	NULL	NULL	regulatory molecules	GP		blocks		physically			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_40_39251_s_212	12882979	3 Alternatively, mechanisms to inhibit FADD and procaspase-8 binding to TRADD may exist, either by regulatory molecules physically blocking this association or preferentially enhancing the TRAF2 and RIP binding to TRADD.	bind
29065	2	7593	5	13	NULL	NULL	NULL	FADD	GP		bind					TRADD	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_40_39251_s_212	12882979	3 Alternatively, mechanisms to inhibit FADD and procaspase-8 binding to TRADD may exist, either by regulatory molecules physically blocking this association or preferentially enhancing the TRAF2 and RIP binding to TRADD.	bind
29066	4	7593	5	13	NULL	NULL	NULL	regulatory molecules	GP		blocks		physically			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_40_39251_s_212	12882979	3 Alternatively, mechanisms to inhibit FADD and procaspase-8 binding to TRADD may exist, either by regulatory molecules physically blocking this association or preferentially enhancing the TRAF2 and RIP binding to TRADD.	bind
29067	5	7593	5	13	NULL	NULL	NULL	TRAF2	GP		bind					TRADD	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_40_39251_s_212	12882979	3 Alternatively, mechanisms to inhibit FADD and procaspase-8 binding to TRADD may exist, either by regulatory molecules physically blocking this association or preferentially enhancing the TRAF2 and RIP binding to TRADD.	bind
29068	6	7593	5	13	NULL	NULL	NULL	RIP	GP		bind					TRADD	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_40_39251_s_212	12882979	3 Alternatively, mechanisms to inhibit FADD and procaspase-8 binding to TRADD may exist, either by regulatory molecules physically blocking this association or preferentially enhancing the TRAF2 and RIP binding to TRADD.	bind
29069	7	7593	5	13	NULL	NULL	NULL	statement 5	Process	enhancing	inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_40_39251_s_212	12882979	3 Alternatively, mechanisms to inhibit FADD and procaspase-8 binding to TRADD may exist, either by regulatory molecules physically blocking this association or preferentially enhancing the TRAF2 and RIP binding to TRADD.	bind
29070	8	7593	5	13	NULL	NULL	NULL	statement 5	Process	enhancing	inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_40_39251_s_212	12882979	3 Alternatively, mechanisms to inhibit FADD and procaspase-8 binding to TRADD may exist, either by regulatory molecules physically blocking this association or preferentially enhancing the TRAF2 and RIP binding to TRADD.	bind
29071	9	7593	5	13	NULL	NULL	NULL	statement 6	Process	enhancing	inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_40_39251_s_212	12882979	3 Alternatively, mechanisms to inhibit FADD and procaspase-8 binding to TRADD may exist, either by regulatory molecules physically blocking this association or preferentially enhancing the TRAF2 and RIP binding to TRADD.	bind
29072	10	7593	5	13	NULL	NULL	NULL	statement 6	Process	enhancing	inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_40_39251_s_212	12882979	3 Alternatively, mechanisms to inhibit FADD and procaspase-8 binding to TRADD may exist, either by regulatory molecules physically blocking this association or preferentially enhancing the TRAF2 and RIP binding to TRADD.	bind
31300	1	7593	7	NULL	NULL	0	NULL	FADD	NULL		bind	NULL				TRADD	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_40_39251_s_212	12882979	3 Alternatively, mechanisms to inhibit FADD and procaspase-8 binding to TRADD may exist, either by regulatory molecules physically blocking this association or preferentially enhancing the TRAF2 and RIP binding to TRADD.	bind
31301	2	7593	7	NULL	NULL	0	NULL	procaspase-8	NULL		bind	NULL				TRADD	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_40_39251_s_212	12882979	3 Alternatively, mechanisms to inhibit FADD and procaspase-8 binding to TRADD may exist, either by regulatory molecules physically blocking this association or preferentially enhancing the TRAF2 and RIP binding to TRADD.	bind
31302	3	7593	7	10	NULL	0	NULL	regulatory molecules			block		physically			statement 1					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_40_39251_s_212	12882979	3 Alternatively, mechanisms to inhibit FADD and procaspase-8 binding to TRADD may exist, either by regulatory molecules physically blocking this association or preferentially enhancing the TRAF2 and RIP binding to TRADD.	bind
31303	4	7593	7	10	NULL	0	NULL	regulatory molecules			block		physically			statement 2					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_40_39251_s_212	12882979	3 Alternatively, mechanisms to inhibit FADD and procaspase-8 binding to TRADD may exist, either by regulatory molecules physically blocking this association or preferentially enhancing the TRAF2 and RIP binding to TRADD.	bind
31304	5	7593	7	NULL	NULL	0	NULL	TRAF2	NULL		bind	NULL				TRADD	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_40_39251_s_212	12882979	3 Alternatively, mechanisms to inhibit FADD and procaspase-8 binding to TRADD may exist, either by regulatory molecules physically blocking this association or preferentially enhancing the TRAF2 and RIP binding to TRADD.	bind
31305	6	7593	7	NULL	NULL	0	NULL	RIP	NULL		bind	NULL				TRADD	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_40_39251_s_212	12882979	3 Alternatively, mechanisms to inhibit FADD and procaspase-8 binding to TRADD may exist, either by regulatory molecules physically blocking this association or preferentially enhancing the TRAF2 and RIP binding to TRADD.	bind
31306	7	7593	7	NULL	NULL	0	NULL	statement 5	NULL	enhancement of	inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_40_39251_s_212	12882979	3 Alternatively, mechanisms to inhibit FADD and procaspase-8 binding to TRADD may exist, either by regulatory molecules physically blocking this association or preferentially enhancing the TRAF2 and RIP binding to TRADD.	bind
31307	8	7593	7	NULL	NULL	0	NULL	statement 5	NULL	enhancement of	inhibits	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_40_39251_s_212	12882979	3 Alternatively, mechanisms to inhibit FADD and procaspase-8 binding to TRADD may exist, either by regulatory molecules physically blocking this association or preferentially enhancing the TRAF2 and RIP binding to TRADD.	bind
31308	9	7593	7	NULL	NULL	0	NULL	statement 6	NULL	enhancement of	inhibits	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_40_39251_s_212	12882979	3 Alternatively, mechanisms to inhibit FADD and procaspase-8 binding to TRADD may exist, either by regulatory molecules physically blocking this association or preferentially enhancing the TRAF2 and RIP binding to TRADD.	bind
31309	10	7593	7	NULL	NULL	0	NULL	statement 6	NULL	enhancement of	inhibits	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_40_39251_s_212	12882979	3 Alternatively, mechanisms to inhibit FADD and procaspase-8 binding to TRADD may exist, either by regulatory molecules physically blocking this association or preferentially enhancing the TRAF2 and RIP binding to TRADD.	bind
29833	1	7594	5	13	NULL	NULL	NULL	Arix	GP		bind					DB1	GP			enhancer	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_4_2911_s_351	10644760	3 Alternatively, the binding of Arix to the DB1 enhancer may provide a favorable environment for the recruitment of Fos-Jun heterodimers to the CRE/AP1 site following PKA stimulation.	bind
29834	2	7594	5	13	NULL	NULL	NULL	Fos-Jun heterodimers	GP		is recruited to									CRE/AP1 site	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_4_2911_s_351	10644760	3 Alternatively, the binding of Arix to the DB1 enhancer may provide a favorable environment for the recruitment of Fos-Jun heterodimers to the CRE/AP1 site following PKA stimulation.	bind
29835	3	7594	5	13	NULL	NULL	NULL	statement 2	Process		occurs following					PKA	GP	stimulation with			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_4_2911_s_351	10644760	3 Alternatively, the binding of Arix to the DB1 enhancer may provide a favorable environment for the recruitment of Fos-Jun heterodimers to the CRE/AP1 site following PKA stimulation.	bind
29836	4	7594	5	13	NULL	NULL	NULL	statement 1	Process		provide		may			statement 3	Process	favorable environment for			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_4_2911_s_351	10644760	3 Alternatively, the binding of Arix to the DB1 enhancer may provide a favorable environment for the recruitment of Fos-Jun heterodimers to the CRE/AP1 site following PKA stimulation.	bind
31310	1	7594	7	NULL	NULL	0	NULL	 Arix	NULL		bind	NULL				DB1	NULL			enhancer	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_4_2911_s_351	10644760	3 Alternatively, the binding of Arix to the DB1 enhancer may provide a favorable environment for the recruitment of Fos-Jun heterodimers to the CRE/AP1 site following PKA stimulation.	bind
31311	2	7594	7	10	NULL	0	NULL	Fos-Jun heterodimers 			is recruited to									CRE/AP1 site 	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_4_2911_s_351	10644760	3 Alternatively, the binding of Arix to the DB1 enhancer may provide a favorable environment for the recruitment of Fos-Jun heterodimers to the CRE/AP1 site following PKA stimulation.	bind
31312	3	7594	7	NULL	NULL	0	NULL	statement 2	NULL		occurs upon	NULL				PKA	NULL	stimulation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_4_2911_s_351	10644760	3 Alternatively, the binding of Arix to the DB1 enhancer may provide a favorable environment for the recruitment of Fos-Jun heterodimers to the CRE/AP1 site following PKA stimulation.	bind
31313	4	7594	7	NULL	NULL	0	NULL	statement 1	NULL		favor	NULL	may			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_4_2911_s_351	10644760	3 Alternatively, the binding of Arix to the DB1 enhancer may provide a favorable environment for the recruitment of Fos-Jun heterodimers to the CRE/AP1 site following PKA stimulation.	bind
29073	1	7595	5	13	NULL	NULL	NULL	SP-A	GP		bind		directly			TLR4	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_31_21771_s_322	16754682	3 Although further experiments are required, we speculate that the physiological meaning of the direct binding of SP-A to TLR4 may be to modulate the subsequent structural changes of TLR4 initiated by LPS binding to MD-2.	bind
29074	2	7595	5	13	NULL	NULL	NULL	LPS	Chemical		bind					MD-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_31_21771_s_322	16754682	3 Although further experiments are required, we speculate that the physiological meaning of the direct binding of SP-A to TLR4 may be to modulate the subsequent structural changes of TLR4 initiated by LPS binding to MD-2.	bind
29075	3	7595	5	13	NULL	NULL	NULL	TLR4	GP	structural changes of	is initiated by					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_31_21771_s_322	16754682	3 Although further experiments are required, we speculate that the physiological meaning of the direct binding of SP-A to TLR4 may be to modulate the subsequent structural changes of TLR4 initiated by LPS binding to MD-2.	bind
29076	4	7595	5	13	NULL	NULL	NULL	statement 1	Process		modulate		may			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_31_21771_s_322	16754682	3 Although further experiments are required, we speculate that the physiological meaning of the direct binding of SP-A to TLR4 may be to modulate the subsequent structural changes of TLR4 initiated by LPS binding to MD-2.	bind
31314	1	7595	7	NULL	NULL	0	NULL	 SP-A	NULL		bind	NULL				TLR4	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_31_21771_s_322	16754682	3 Although further experiments are required, we speculate that the physiological meaning of the direct binding of SP-A to TLR4 may be to modulate the subsequent structural changes of TLR4 initiated by LPS binding to MD-2.	bind
31315	2	7595	7	NULL	NULL	0	NULL	LPS	NULL		bind	NULL				MD-2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_31_21771_s_322	16754682	3 Although further experiments are required, we speculate that the physiological meaning of the direct binding of SP-A to TLR4 may be to modulate the subsequent structural changes of TLR4 initiated by LPS binding to MD-2.	bind
31316	3	7595	7	NULL	NULL	0	NULL	statement 2	NULL		initiate	NULL				TLR4	NULL	structural changes of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_31_21771_s_322	16754682	3 Although further experiments are required, we speculate that the physiological meaning of the direct binding of SP-A to TLR4 may be to modulate the subsequent structural changes of TLR4 initiated by LPS binding to MD-2.	bind
31317	4	7595	7	NULL	NULL	0	NULL	statement 1	NULL		modulate	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_31_21771_s_322	16754682	3 Although further experiments are required, we speculate that the physiological meaning of the direct binding of SP-A to TLR4 may be to modulate the subsequent structural changes of TLR4 initiated by LPS binding to MD-2.	bind
54562	1	7596	5	13	NULL	NULL	NULL				bind			CUT domain		DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_8_5319_s_21	16371359	3 Although this structure showed similarity to those of the POU-specific domains of POU-homologous proteins ( ,  ), the DNA-binding mechanism of the CUT domain is yet unknown.	bind
31318	1	7596	7	NULL	NULL	0	NULL		NULL		bind	NULL		CUT domain		DNA	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_8_5319_s_21	16371359	3 Although this structure showed similarity to those of the POU-specific domains of POU-homologous proteins ( ,  ), the DNA-binding mechanism of the CUT domain is yet unknown.	bind
29077	2	7598	5	13	NULL	NULL	NULL	statement 1	GP		bind					Galpha(GDP)	GP	inactive			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_45_38071_s_11	16129667	3 An agonist-activated GPCR (R*) binds to the inactive Galpha(GDP).	bind
54563	1	7598	5	13	NULL	NULL	NULL	agonist	Chemical		activates					GPCR (R*)	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_45_38071_s_11	16129667	3 An agonist-activated GPCR (R*) binds to the inactive Galpha(GDP).	bind
31320	1	7598	7	NULL	NULL	0	NULL	agonist	NULL		activates	NULL				GPCR (R*)	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_45_38071_s_11	16129667	3 An agonist-activated GPCR (R*) binds to the inactive Galpha(GDP).	bind
31321	2	7598	7	NULL	NULL	0	NULL	statement 1	NULL		binds to	NULL				Galpha(GDP)	NULL	inactive			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_45_38071_s_11	16129667	3 An agonist-activated GPCR (R*) binds to the inactive Galpha(GDP).	bind
29079	1	7599	5	13	NULL	NULL	NULL	SHBG	GP		does not bind					C4BP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_23_14658_s_44	9169428	3 and  4) bind to human C4BP with about the same affinity, whereas the homologous proteins SHBG (26% identical to the SHBG-like domain of human protein S; see Ref.  38) and growth arrest-specific protein 6 (Gas 6) (44% identical to human protein S; see Ref.  39) do not show any detectable binding to C4BP.	bind
29080	2	7599	5	13	NULL	NULL	NULL	Gas 6	GP		is					growth arrest-specific protein 6	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_23_14658_s_44	9169428	3 and  4) bind to human C4BP with about the same affinity, whereas the homologous proteins SHBG (26% identical to the SHBG-like domain of human protein S; see Ref.  38) and growth arrest-specific protein 6 (Gas 6) (44% identical to human protein S; see Ref.  39) do not show any detectable binding to C4BP.	bind
29081	3	7599	5	13	NULL	NULL	NULL	Gas 6	GP		does not bind					C4BP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_23_14658_s_44	9169428	3 and  4) bind to human C4BP with about the same affinity, whereas the homologous proteins SHBG (26% identical to the SHBG-like domain of human protein S; see Ref.  38) and growth arrest-specific protein 6 (Gas 6) (44% identical to human protein S; see Ref.  39) do not show any detectable binding to C4BP.	bind
46665	4	7599	5	13	NULL	NULL	NULL	SHBG	GP		is similar to					protein S	GP	human	SHBG-like domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_23_14658_s_44	9169428	3 and  4) bind to human C4BP with about the same affinity, whereas the homologous proteins SHBG (26% identical to the SHBG-like domain of human protein S; see Ref.  38) and growth arrest-specific protein 6 (Gas 6) (44% identical to human protein S; see Ref.  39) do not show any detectable binding to C4BP.	bind
46666	5	7599	5	13	NULL	NULL	NULL	Gas 6	GP		is similar to					protein S	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_23_14658_s_44	9169428	3 and  4) bind to human C4BP with about the same affinity, whereas the homologous proteins SHBG (26% identical to the SHBG-like domain of human protein S; see Ref.  38) and growth arrest-specific protein 6 (Gas 6) (44% identical to human protein S; see Ref.  39) do not show any detectable binding to C4BP.	bind
31322	1	7599	7	NULL	NULL	0	NULL	SHBG	NULL		is identical to	NULL				protein S	NULL	human	SHBG-like domain 		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_23_14658_s_44	9169428	3 and  4) bind to human C4BP with about the same affinity, whereas the homologous proteins SHBG (26% identical to the SHBG-like domain of human protein S; see Ref.  38) and growth arrest-specific protein 6 (Gas 6) (44% identical to human protein S; see Ref.  39) do not show any detectable binding to C4BP.	bind
31323	2	7599	7	NULL	NULL	0	NULL	Gas 6	NULL		is identical to	NULL				protein S	NULL	human			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_23_14658_s_44	9169428	3 and  4) bind to human C4BP with about the same affinity, whereas the homologous proteins SHBG (26% identical to the SHBG-like domain of human protein S; see Ref.  38) and growth arrest-specific protein 6 (Gas 6) (44% identical to human protein S; see Ref.  39) do not show any detectable binding to C4BP.	bind
31324	3	7599	7	NULL	NULL	0	NULL	SHBG	NULL		does not bind	NULL				C4BP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_23_14658_s_44	9169428	3 and  4) bind to human C4BP with about the same affinity, whereas the homologous proteins SHBG (26% identical to the SHBG-like domain of human protein S; see Ref.  38) and growth arrest-specific protein 6 (Gas 6) (44% identical to human protein S; see Ref.  39) do not show any detectable binding to C4BP.	bind
31325	4	7599	7	NULL	NULL	0	NULL	Gas 6	NULL		does not bind	NULL				C4BP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_23_14658_s_44	9169428	3 and  4) bind to human C4BP with about the same affinity, whereas the homologous proteins SHBG (26% identical to the SHBG-like domain of human protein S; see Ref.  38) and growth arrest-specific protein 6 (Gas 6) (44% identical to human protein S; see Ref.  39) do not show any detectable binding to C4BP.	bind
31326	5	7599	7	NULL	NULL	0	NULL	Gas 6	NULL		is	NULL				growth arrest-specific protein 6 	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_23_14658_s_44	9169428	3 and  4) bind to human C4BP with about the same affinity, whereas the homologous proteins SHBG (26% identical to the SHBG-like domain of human protein S; see Ref.  38) and growth arrest-specific protein 6 (Gas 6) (44% identical to human protein S; see Ref.  39) do not show any detectable binding to C4BP.	bind
29082	1	7600	5	13	NULL	NULL	NULL	anti-N antibodies	GP		bind					ez1-586	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_20088_s_192	9242682	3 Anti-N and anti-C antibodies bound both ez1-586 and ez1-333.	bind
29083	2	7600	5	13	NULL	NULL	NULL	anti-N antibodies	GP		bind					ez1-333	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_20088_s_192	9242682	3 Anti-N and anti-C antibodies bound both ez1-586 and ez1-333.	bind
29084	3	7600	5	13	NULL	NULL	NULL	anti-C antibodies	GP		bind					ez1-586	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_20088_s_192	9242682	3 Anti-N and anti-C antibodies bound both ez1-586 and ez1-333.	bind
29085	4	7600	5	13	NULL	NULL	NULL	anti-C antibodies	GP		bind					ez1-333	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_20088_s_192	9242682	3 Anti-N and anti-C antibodies bound both ez1-586 and ez1-333.	bind
31327	1	7600	7	NULL	NULL	0	NULL	Anti-N antibody	NULL		bind	NULL				 ez1-586	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_32_20088_s_192	9242682	3 Anti-N and anti-C antibodies bound both ez1-586 and ez1-333.	bind
31328	2	7600	7	NULL	NULL	0	NULL	anti-C antibody	NULL		bind	NULL				ez1-333	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_32_20088_s_192	9242682	3 Anti-N and anti-C antibodies bound both ez1-586 and ez1-333.	bind
46586	3	7600	7	10	NULL	0	NULL	anti-C antibody	NULL		bind	NULL				ez1-586	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_20088_s_192	9242682	3 Anti-N and anti-C antibodies bound both ez1-586 and ez1-333.	bind
46587	1	7600	7	10	NULL	0	NULL	Anti-N antibody	NULL		bind	NULL				 ez1-333	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_32_20088_s_192	9242682	3 Anti-N and anti-C antibodies bound both ez1-586 and ez1-333.	bind
29123	1	7601	5	13	NULL	NULL	NULL	TNFalpha	GP		bind					membrane receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_23_13333_s_212	8662837	3 As the protective capabilities of M-T2 correlate with its ability to inhibit binding of TNFalpha to membrane receptors, we conclude that M-T2 inhibits the cytolytic activities of TNFalpha by physically preventing TNFalpha from associating with its cognate TNF membrane receptors.	bind
29124	2	7601	5	13	NULL	NULL	NULL	M-T2	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_23_13333_s_212	8662837	3 As the protective capabilities of M-T2 correlate with its ability to inhibit binding of TNFalpha to membrane receptors, we conclude that M-T2 inhibits the cytolytic activities of TNFalpha by physically preventing TNFalpha from associating with its cognate TNF membrane receptors.	bind
29125	3	7601	5	13	NULL	NULL	NULL	TNFalpha	GP		associates with					TNF membrane receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_23_13333_s_212	8662837	3 As the protective capabilities of M-T2 correlate with its ability to inhibit binding of TNFalpha to membrane receptors, we conclude that M-T2 inhibits the cytolytic activities of TNFalpha by physically preventing TNFalpha from associating with its cognate TNF membrane receptors.	bind
29126	4	7601	5	13	NULL	NULL	NULL	M-T2	GP		prevents		physically			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_23_13333_s_212	8662837	3 As the protective capabilities of M-T2 correlate with its ability to inhibit binding of TNFalpha to membrane receptors, we conclude that M-T2 inhibits the cytolytic activities of TNFalpha by physically preventing TNFalpha from associating with its cognate TNF membrane receptors.	bind
29127	5	7601	5	13	NULL	NULL	NULL	TNFalpha	GP		exhibits					cytolytic activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_23_13333_s_212	8662837	3 As the protective capabilities of M-T2 correlate with its ability to inhibit binding of TNFalpha to membrane receptors, we conclude that M-T2 inhibits the cytolytic activities of TNFalpha by physically preventing TNFalpha from associating with its cognate TNF membrane receptors.	bind
46653	6	7601	5	13	NULL	NULL	NULL	M-T2	GP		inhibits					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_23_13333_s_212	8662837	3 As the protective capabilities of M-T2 correlate with its ability to inhibit binding of TNFalpha to membrane receptors, we conclude that M-T2 inhibits the cytolytic activities of TNFalpha by physically preventing TNFalpha from associating with its cognate TNF membrane receptors.	bind
23187	1	7601	6	NULL	NULL	0	NULL	TNFalpha	NULL		bind	NULL				membrane receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_23_13333_s_212	8662837	3 As the protective capabilities of M-T2 correlate with its ability to inhibit binding of TNFalpha to membrane receptors, we conclude that M-T2 inhibits the cytolytic activities of TNFalpha by physically preventing TNFalpha from associating with its cognate TNF membrane receptors.	bind
23188	2	7601	6	NULL	NULL	0	NULL	M-T2 	NULL		inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_23_13333_s_212	8662837	3 As the protective capabilities of M-T2 correlate with its ability to inhibit binding of TNFalpha to membrane receptors, we conclude that M-T2 inhibits the cytolytic activities of TNFalpha by physically preventing TNFalpha from associating with its cognate TNF membrane receptors.	bind
23189	3	7601	6	NULL	NULL	0	NULL	TNFalpha	NULL		exhibit	NULL				cytolytic activities	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_23_13333_s_212	8662837	3 As the protective capabilities of M-T2 correlate with its ability to inhibit binding of TNFalpha to membrane receptors, we conclude that M-T2 inhibits the cytolytic activities of TNFalpha by physically preventing TNFalpha from associating with its cognate TNF membrane receptors.	bind
23190	4	7601	6	NULL	NULL	0	NULL	M-T2	NULL		inhibit	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_23_13333_s_212	8662837	3 As the protective capabilities of M-T2 correlate with its ability to inhibit binding of TNFalpha to membrane receptors, we conclude that M-T2 inhibits the cytolytic activities of TNFalpha by physically preventing TNFalpha from associating with its cognate TNF membrane receptors.	bind
23191	5	7601	6	NULL	NULL	0	NULL	TNFalpha	NULL		associate with	NULL				TNF membrane receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_23_13333_s_212	8662837	3 As the protective capabilities of M-T2 correlate with its ability to inhibit binding of TNFalpha to membrane receptors, we conclude that M-T2 inhibits the cytolytic activities of TNFalpha by physically preventing TNFalpha from associating with its cognate TNF membrane receptors.	bind
23270	6	7601	6	NULL	NULL	0	NULL	M-T2	NULL		inhibits	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_23_13333_s_212	8662837	3 As the protective capabilities of M-T2 correlate with its ability to inhibit binding of TNFalpha to membrane receptors, we conclude that M-T2 inhibits the cytolytic activities of TNFalpha by physically preventing TNFalpha from associating with its cognate TNF membrane receptors.	bind
29129	1	7602	5	13	NULL	NULL	NULL	p130Cas	GP		bind		consistently	SH3 domain		PTP1B	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_49_31290_s_86	8940134	3 As the SH3 domain derived from p130Cas consistently bound more PTP1B than any other SH3 domain tested  in vitro (as assessed by densitometry of immunoblots), we investigated this interaction in more detail.	bind
23272	1	7602	6	NULL	NULL	0	NULL	p130Cas	NULL		bind	NULL	consistently	SH3 domain		PTP1B	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_271_49_31290_s_86	8940134	3 As the SH3 domain derived from p130Cas consistently bound more PTP1B than any other SH3 domain tested  in vitro (as assessed by densitometry of immunoblots), we investigated this interaction in more detail.	bind
29130	1	7604	5	13	NULL	NULL	NULL	vitronectin	GP		bind					fibrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_26_19788_s_29	10764803	3 Based on these observations, we hypothesized that fibrin-bound vitronectin supports PAI-1 binding.	bind
29132	2	7604	5	13	NULL	NULL	NULL	statement 1	Process		supports					PAI-1	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_26_19788_s_29	10764803	3 Based on these observations, we hypothesized that fibrin-bound vitronectin supports PAI-1 binding.	bind
23281	1	7604	6	NULL	NULL	0	NULL	fibrin	NULL		bind	NULL				vitronectin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_26_19788_s_29	10764803	3 Based on these observations, we hypothesized that fibrin-bound vitronectin supports PAI-1 binding.	bind
23282	2	7604	6	NULL	NULL	0	NULL	statement 1	NULL		supports	NULL				PAI-1	NULL	binding of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_26_19788_s_29	10764803	3 Based on these observations, we hypothesized that fibrin-bound vitronectin supports PAI-1 binding.	bind
29133	1	7605	5	13	NULL	NULL	NULL	IMP	Chemical		bind					synthetase	GP		GTP pocket		NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_30_26779_s_271	12004071	3 Because IMP concentrations in exhaustively exercised muscle rise to 3.6 mM ( 12), the binding of IMP to the GTP pocket of the synthetase may occur  in vivo under these conditions.	bind
29136	2	7605	5	13	NULL	NULL	NULL	IMP	Chemical		rise in					muscle	OrganismPart	exhaustively exercised			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_30_26779_s_271	12004071	3 Because IMP concentrations in exhaustively exercised muscle rise to 3.6 mM ( 12), the binding of IMP to the GTP pocket of the synthetase may occur  in vivo under these conditions.	bind
23290	1	7605	6	NULL	NULL	0	NULL	IMP	NULL		bind	NULL	may			synthetase	NULL		GTP pocket		NULL	in vivo	0	NULL	NULL	NULL	gw60_jbiolchem_277_30_26779_s_271	12004071	3 Because IMP concentrations in exhaustively exercised muscle rise to 3.6 mM ( 12), the binding of IMP to the GTP pocket of the synthetase may occur  in vivo under these conditions.	bind
29137	1	7606	5	13	NULL	NULL	NULL	rigor myosin	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_8_982_s_54	15302786	3 Before each experiment, myosin (200 mug/mL), equimolar actin, and 1 mmol/L ATP are centrifuged (320 000 g; 20 minutes) to remove noncycling, rigor myosin bound to actin.	bind
23295	1	7606	6	NULL	NULL	0	NULL	rigor myosin	NULL		bind	NULL				actin	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_110_8_982_s_54	15302786	3 Before each experiment, myosin (200 mug/mL), equimolar actin, and 1 mmol/L ATP are centrifuged (320 000 g; 20 minutes) to remove noncycling, rigor myosin bound to actin.	bind
29138	1	7607	5	13	NULL	NULL	NULL	Rac isoforms	GP		bind					p67 phox	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_30_18834_s_166	9228059	3 Binding of Rac isoforms to p67 phox has been demonstrated using p67 phox (or a p67 phox-GST fusion protein) immobilized on glutathione beads ( 46) or on a nitrocellulose filter ( 48,  60) and also by yeast two-hybrid analysis ( 49).	bind
23296	1	7607	6	NULL	NULL	0	NULL	Rac isoforms	NULL		bind	NULL				p67 phox	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_30_18834_s_166	9228059	3 Binding of Rac isoforms to p67 phox has been demonstrated using p67 phox (or a p67 phox-GST fusion protein) immobilized on glutathione beads ( 46) or on a nitrocellulose filter ( 48,  60) and also by yeast two-hybrid analysis ( 49).	bind
29141	1	7609	5	13	NULL	NULL	NULL	Rsp5p	GP		is a type of			WW domains					type I WW domains		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_28_25974_s_251	11356856	3 Chang  et al. ( 58) showed that Rsp5p WW domains are type I WW domains that bind preferentially to PP XY-containing ligands.	bind
29147	2	7609	5	13	NULL	NULL	NULL	statement 1	GP		bind		preferentially			PP XY-containing ligands	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_28_25974_s_251	11356856	3 Chang  et al. ( 58) showed that Rsp5p WW domains are type I WW domains that bind preferentially to PP XY-containing ligands.	bind
23300	1	7609	6	10	NULL	0	NULL	Rsp5p	NULL		is a type of	NULL		WW domain			NULL		type I WW domains		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_28_25974_s_251	11356856	3 Chang  et al. ( 58) showed that Rsp5p WW domains are type I WW domains that bind preferentially to PP XY-containing ligands.	bind
23301	2	7609	6	NULL	NULL	0	NULL	Rsp5p	NULL		bind	NULL	preferentially	WW domain		PP-XY containing ligands	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_28_25974_s_251	11356856	3 Chang  et al. ( 58) showed that Rsp5p WW domains are type I WW domains that bind preferentially to PP XY-containing ligands.	bind
29150	1	7610	5	13	NULL	NULL	NULL	MyHC	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_18_2276_s_11	15883223	3 Consequently, MyHC binds to actin, hydrolyzes ATP to adenosine diphosphate (ADP) and inorganic phosphate, and displaces the actin filament.	bind
29157	2	7610	5	13	NULL	NULL	NULL	ATP	Chemical		is hydrolysed to					ADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_18_2276_s_11	15883223	3 Consequently, MyHC binds to actin, hydrolyzes ATP to adenosine diphosphate (ADP) and inorganic phosphate, and displaces the actin filament.	bind
29159	3	7610	5	13	NULL	NULL	NULL	statement 2	Process		displaces					actin filament	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_18_2276_s_11	15883223	3 Consequently, MyHC binds to actin, hydrolyzes ATP to adenosine diphosphate (ADP) and inorganic phosphate, and displaces the actin filament.	bind
29160	4	7610	5	13	NULL	NULL	NULL	ADP	Chemical		is					adenosine diphosphate	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_18_2276_s_11	15883223	3 Consequently, MyHC binds to actin, hydrolyzes ATP to adenosine diphosphate (ADP) and inorganic phosphate, and displaces the actin filament.	bind
55525	5	7610	5	13	NULL	NULL	NULL	ATP	Chemical		is hydrolyzed to					inorganic phosphate	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_18_2276_s_11	15883223	3 Consequently, MyHC binds to actin, hydrolyzes ATP to adenosine diphosphate (ADP) and inorganic phosphate, and displaces the actin filament.	bind
55526	6	7610	5	13	NULL	NULL	NULL	statement 2	Process		occurs along with					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_18_2276_s_11	15883223	3 Consequently, MyHC binds to actin, hydrolyzes ATP to adenosine diphosphate (ADP) and inorganic phosphate, and displaces the actin filament.	bind
23302	1	7610	6	NULL	NULL	0	NULL	MyHC	NULL		bind	NULL				actin	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_111_18_2276_s_11	15883223	3 Consequently, MyHC binds to actin, hydrolyzes ATP to adenosine diphosphate (ADP) and inorganic phosphate, and displaces the actin filament.	bind
23303	2	7610	6	NULL	NULL	0	NULL	MyHC	NULL		displaces 	NULL				actin filament	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_111_18_2276_s_11	15883223	3 Consequently, MyHC binds to actin, hydrolyzes ATP to adenosine diphosphate (ADP) and inorganic phosphate, and displaces the actin filament.	bind
23304	3	7610	6	10	NULL	0	NULL	ATP			hydrolyzed to					ADP					NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_18_2276_s_11	15883223	3 Consequently, MyHC binds to actin, hydrolyzes ATP to adenosine diphosphate (ADP) and inorganic phosphate, and displaces the actin filament.	bind
23305	4	7610	6	NULL	NULL	0	NULL	MyHC	NULL		plays a role in	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_111_18_2276_s_11	15883223	3 Consequently, MyHC binds to actin, hydrolyzes ATP to adenosine diphosphate (ADP) and inorganic phosphate, and displaces the actin filament.	bind
46601	5	7610	6	10	NULL	0	NULL	ADP	NULL		is	NULL				adenosine diphosphate	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_111_18_2276_s_11	15883223	3 Consequently, MyHC binds to actin, hydrolyzes ATP to adenosine diphosphate (ADP) and inorganic phosphate, and displaces the actin filament.	bind
55527	6	7610	6	10	NULL	0	NULL	ATP			is hydrolyzed to					inorganic phosphate					NULL		0	NULL	NULL	NULL	gw70_circulation_111_18_2276_s_11	15883223	3 Consequently, MyHC binds to actin, hydrolyzes ATP to adenosine diphosphate (ADP) and inorganic phosphate, and displaces the actin filament.	bind
55528	7	7610	6	10	NULL	0	NULL	statement 3			occurs along with					statement 6					NULL		0	NULL	NULL	NULL	gw70_circulation_111_18_2276_s_11	15883223	3 Consequently, MyHC binds to actin, hydrolyzes ATP to adenosine diphosphate (ADP) and inorganic phosphate, and displaces the actin filament.	bind
30415	1	7611	5	13	NULL	NULL	NULL	oligo FP4	NucleicAcid		bind					nuclear protein	GP	J774 cells			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_12_8331_s_141	10722663	3 Consistent with the footprinting experiments (Fig.  2), oligo FP4 binds a nuclear protein (band F) only from J774 cells.	bind
23306	1	7611	6	10	NULL	0	NULL	oligo FP4			bind					nuclear protein 		J774 cells			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_12_8331_s_141	10722663	3 Consistent with the footprinting experiments (Fig.  2), oligo FP4 binds a nuclear protein (band F) only from J774 cells.	bind
30416	1	7612	5	13	NULL	NULL	NULL	CT-1	GP		bind					gp130	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_2_128_s_23	11834704	3 CT-1 binds to glycoprotein130 (gp130) and the leukemia inhibitory factor (LIF) receptor, a component of the gp130 receptor.	bind
30417	2	7612	5	13	NULL	NULL	NULL	gp130	GP		is					glycoprotein130	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_2_128_s_23	11834704	3 CT-1 binds to glycoprotein130 (gp130) and the leukemia inhibitory factor (LIF) receptor, a component of the gp130 receptor.	bind
30418	3	7612	5	13	NULL	NULL	NULL	CT-1	GP		bind					LIF receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_2_128_s_23	11834704	3 CT-1 binds to glycoprotein130 (gp130) and the leukemia inhibitory factor (LIF) receptor, a component of the gp130 receptor.	bind
30419	4	7612	5	13	NULL	NULL	NULL	LIF receptor	GP		is					leukemia inhibitory factor receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_2_128_s_23	11834704	3 CT-1 binds to glycoprotein130 (gp130) and the leukemia inhibitory factor (LIF) receptor, a component of the gp130 receptor.	bind
30420	5	7612	5	13	NULL	NULL	NULL	LIF receptor	GP		is a component of					gp130 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_2_128_s_23	11834704	3 CT-1 binds to glycoprotein130 (gp130) and the leukemia inhibitory factor (LIF) receptor, a component of the gp130 receptor.	bind
23307	1	7612	6	NULL	NULL	0	NULL	CT-1	NULL		bind	NULL				gp130	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_2_128_s_23	11834704	3 CT-1 binds to glycoprotein130 (gp130) and the leukemia inhibitory factor (LIF) receptor, a component of the gp130 receptor.	bind
23308	2	7612	6	NULL	NULL	0	NULL	gp130	NULL		is	NULL				glycoprotein130	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_2_128_s_23	11834704	3 CT-1 binds to glycoprotein130 (gp130) and the leukemia inhibitory factor (LIF) receptor, a component of the gp130 receptor.	bind
23309	3	7612	6	NULL	NULL	0	NULL	CT-1	NULL		bind	NULL				LIF receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_2_128_s_23	11834704	3 CT-1 binds to glycoprotein130 (gp130) and the leukemia inhibitory factor (LIF) receptor, a component of the gp130 receptor.	bind
23310	4	7612	6	NULL	NULL	0	NULL	LIF	NULL		is	NULL				leukemia inhibitory factor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_2_128_s_23	11834704	3 CT-1 binds to glycoprotein130 (gp130) and the leukemia inhibitory factor (LIF) receptor, a component of the gp130 receptor.	bind
23311	5	7612	6	NULL	NULL	0	NULL	LIF receptor	NULL		is a component of	NULL				gp130 receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_2_128_s_23	11834704	3 CT-1 binds to glycoprotein130 (gp130) and the leukemia inhibitory factor (LIF) receptor, a component of the gp130 receptor.	bind
30421	1	7613	5	13	NULL	NULL	NULL	Myc-Raf	GP		bind					GST-14.3.3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_40_23681_s_267	7559537	3 dimerization, inasmuch as the Myc-Raf  bound to GST-14.3.3 (1-180) ( Fig. 5 C,  middle panel,  lane 5), which dimerizes quite  well with Myc-14.3.3 ( Fig. 5 B,  bottom panel,  lane 5), also lacks detectable  kinase activity ( Fig. 5 C,  bottom panel,  lane 5).	bind
30422	2	7613	5	13	NULL	NULL	NULL	GST-14.3.3	GP		dimerizes with					Myc-14.3.3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_40_23681_s_267	7559537	3 dimerization, inasmuch as the Myc-Raf  bound to GST-14.3.3 (1-180) ( Fig. 5 C,  middle panel,  lane 5), which dimerizes quite  well with Myc-14.3.3 ( Fig. 5 B,  bottom panel,  lane 5), also lacks detectable  kinase activity ( Fig. 5 C,  bottom panel,  lane 5).	bind
30423	3	7613	5	13	NULL	NULL	NULL	GST-14.3.3	GP		lacks					kinase activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_40_23681_s_267	7559537	3 dimerization, inasmuch as the Myc-Raf  bound to GST-14.3.3 (1-180) ( Fig. 5 C,  middle panel,  lane 5), which dimerizes quite  well with Myc-14.3.3 ( Fig. 5 B,  bottom panel,  lane 5), also lacks detectable  kinase activity ( Fig. 5 C,  bottom panel,  lane 5).	bind
23312	1	7613	6	NULL	NULL	0	NULL	Myc-Raf	NULL		bind	NULL				GST-14.3.3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_40_23681_s_267	7559537	3 dimerization, inasmuch as the Myc-Raf  bound to GST-14.3.3 (1-180) ( Fig. 5 C,  middle panel,  lane 5), which dimerizes quite  well with Myc-14.3.3 ( Fig. 5 B,  bottom panel,  lane 5), also lacks detectable  kinase activity ( Fig. 5 C,  bottom panel,  lane 5).	bind
23313	2	7613	6	10	NULL	0	NULL	GST-14.3.3	NULL		dimerizes  with	NULL				Myc-14.3.3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_40_23681_s_267	7559537	3 dimerization, inasmuch as the Myc-Raf  bound to GST-14.3.3 (1-180) ( Fig. 5 C,  middle panel,  lane 5), which dimerizes quite  well with Myc-14.3.3 ( Fig. 5 B,  bottom panel,  lane 5), also lacks detectable  kinase activity ( Fig. 5 C,  bottom panel,  lane 5).	bind
23314	3	7613	6	10	NULL	0	NULL	GST-14.3.3	NULL		lacks	NULL				kinase activity	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_40_23681_s_267	7559537	3 dimerization, inasmuch as the Myc-Raf  bound to GST-14.3.3 (1-180) ( Fig. 5 C,  middle panel,  lane 5), which dimerizes quite  well with Myc-14.3.3 ( Fig. 5 B,  bottom panel,  lane 5), also lacks detectable  kinase activity ( Fig. 5 C,  bottom panel,  lane 5).	bind
30424	1	7614	5	13	NULL	NULL	NULL	Hb	GP	free	bind					Hp	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_1_119_s_16	14656926	3 During intravascular hemolysis, free Hb binds to the plasma protein Hp, and Hb:Hp complexes are formed.	bind
30425	2	7614	5	13	NULL	NULL	NULL	Hp	GP		is a type of					plasma protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_1_119_s_16	14656926	3 During intravascular hemolysis, free Hb binds to the plasma protein Hp, and Hb:Hp complexes are formed.	bind
30426	3	7614	5	13	NULL	NULL	NULL	statement 1	Process		forms					Hb:Hp complexes	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_1_119_s_16	14656926	3 During intravascular hemolysis, free Hb binds to the plasma protein Hp, and Hb:Hp complexes are formed.	bind
30427	4	7614	5	13	NULL	NULL	NULL	statement 1	Process		occurs during					intravascular hemolysis	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_1_119_s_16	14656926	3 During intravascular hemolysis, free Hb binds to the plasma protein Hp, and Hb:Hp complexes are formed.	bind
23315	1	7614	6	10	NULL	0	NULL	Hb		free	bind					Hp					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_1_119_s_16	14656926	3 During intravascular hemolysis, free Hb binds to the plasma protein Hp, and Hb:Hp complexes are formed.	bind
23316	2	7614	6	NULL	NULL	0	NULL	statement 1	NULL		occurs during	NULL				intravascular hemolysis	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_1_119_s_16	14656926	3 During intravascular hemolysis, free Hb binds to the plasma protein Hp, and Hb:Hp complexes are formed.	bind
23317	3	7614	6	NULL	NULL	0	NULL	statement 1	NULL		forms	NULL				Hb:Hp complexes	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_1_119_s_16	14656926	3 During intravascular hemolysis, free Hb binds to the plasma protein Hp, and Hb:Hp complexes are formed.	bind
55529	4	7614	6	10	NULL	0	NULL	Hp			is a type of					plasma protein					NULL		0	NULL	NULL	NULL	gw70_circulationres_94_1_119_s_16	14656926	3 During intravascular hemolysis, free Hb binds to the plasma protein Hp, and Hb:Hp complexes are formed.	bind
30428	1	7615	5	13	NULL	NULL	NULL	Hsp90alpha constructs	GP	recombinant;;chicken	bind			C-terminal		ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_9_7066_s_132	11751878	3 Finally, although we analyzed the binding of rat Hsp90 (beta), Marcu  et al. ( 20) could detect a C-terminal ATP binding by studying ATP-Sepharose binding of recombinant chicken Hsp90alpha constructs.	bind
23318	1	7615	6	10	NULL	0	NULL	Hsp90alpha constructs	NULL	recombinant;;chicken	bind	NULL		C-terminal		ATP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_9_7066_s_132	11751878	3 Finally, although we analyzed the binding of rat Hsp90 (beta), Marcu  et al. ( 20) could detect a C-terminal ATP binding by studying ATP-Sepharose binding of recombinant chicken Hsp90alpha constructs.	bind
30429	1	7616	5	13	NULL	NULL	NULL	MC2R	GP		is a type of					adrenocortical receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_37_23000_s_212	9287296	3 Finally, it is interesting to note that the MC2R, the adrenocortical receptor which only binds the melanocortin ACTH, contains yet a third aspartic acid residue in this region (equivalent to position 118 in hMC1R).	bind
30430	2	7616	5	13	NULL	NULL	NULL	MC2R	GP		bind					ACTH	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_37_23000_s_212	9287296	3 Finally, it is interesting to note that the MC2R, the adrenocortical receptor which only binds the melanocortin ACTH, contains yet a third aspartic acid residue in this region (equivalent to position 118 in hMC1R).	bind
30431	3	7616	5	13	NULL	NULL	NULL	ACTH	GP		is a type of					melanocortin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_37_23000_s_212	9287296	3 Finally, it is interesting to note that the MC2R, the adrenocortical receptor which only binds the melanocortin ACTH, contains yet a third aspartic acid residue in this region (equivalent to position 118 in hMC1R).	bind
30432	4	7616	5	13	NULL	NULL	NULL	MC2R	GP		contains								aspartic acid residue		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_37_23000_s_212	9287296	3 Finally, it is interesting to note that the MC2R, the adrenocortical receptor which only binds the melanocortin ACTH, contains yet a third aspartic acid residue in this region (equivalent to position 118 in hMC1R).	bind
30433	5	7616	5	13	NULL	NULL	NULL	statement 4	AminoAcid		is equivalent to					hMC1R	GP		position 118		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_37_23000_s_212	9287296	3 Finally, it is interesting to note that the MC2R, the adrenocortical receptor which only binds the melanocortin ACTH, contains yet a third aspartic acid residue in this region (equivalent to position 118 in hMC1R).	bind
23323	1	7616	6	10	NULL	0	NULL	MC2R	NULL		bind	NULL				ACTH	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_37_23000_s_212	9287296	3 Finally, it is interesting to note that the MC2R, the adrenocortical receptor which only binds the melanocortin ACTH, contains yet a third aspartic acid residue in this region (equivalent to position 118 in hMC1R).	bind
23325	2	7616	6	10	NULL	0	NULL	MC2R	NULL		contains	NULL					NULL		aspartic acid residue		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_37_23000_s_212	9287296	3 Finally, it is interesting to note that the MC2R, the adrenocortical receptor which only binds the melanocortin ACTH, contains yet a third aspartic acid residue in this region (equivalent to position 118 in hMC1R).	bind
23337	3	7616	6	10	NULL	0	NULL	MC2R	NULL		is equivalent to	NULL		aspartic acid residue		hMC1R	NULL		position 118		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_37_23000_s_212	9287296	3 Finally, it is interesting to note that the MC2R, the adrenocortical receptor which only binds the melanocortin ACTH, contains yet a third aspartic acid residue in this region (equivalent to position 118 in hMC1R).	bind
46620	4	7616	6	10	NULL	0	NULL	MC2R	NULL		is a type of	NULL				adrenocortical receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_37_23000_s_212	9287296	3 Finally, it is interesting to note that the MC2R, the adrenocortical receptor which only binds the melanocortin ACTH, contains yet a third aspartic acid residue in this region (equivalent to position 118 in hMC1R).	bind
46621	5	7616	6	10	NULL	0	NULL	ACTH	NULL		is a type of	NULL				melanocortin 	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_37_23000_s_212	9287296	3 Finally, it is interesting to note that the MC2R, the adrenocortical receptor which only binds the melanocortin ACTH, contains yet a third aspartic acid residue in this region (equivalent to position 118 in hMC1R).	bind
30434	1	7617	5	13	NULL	NULL	NULL	RhoA proteins	GP	stably expressed;;phosphomimetic	bind					Rhotekin	GP		RBD domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_21_19023_s_291	12654918	3 Further,  stably expressed phosphomimetic RhoA proteins bound the RBD domain of the Rho  effector Rhotekin ( Fig.  8 B).	bind
30435	2	7617	5	13	NULL	NULL	NULL	Rhotekin 	GP		is a type of					Rho effector	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_21_19023_s_291	12654918	3 Further,  stably expressed phosphomimetic RhoA proteins bound the RBD domain of the Rho  effector Rhotekin ( Fig.  8 B).	bind
23338	1	7617	6	10	NULL	0	NULL	RhoA protein	NULL	stably expressed;;phosphomimetic 	bind	NULL				Rhotekin	NULL		RBD domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_21_19023_s_291	12654918	3 Further,  stably expressed phosphomimetic RhoA proteins bound the RBD domain of the Rho  effector Rhotekin ( Fig.  8 B).	bind
46622	2	7617	6	10	NULL	0	NULL	Rhotekin	NULL		is a type of	NULL				Rho effector	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_21_19023_s_291	12654918	3 Further,  stably expressed phosphomimetic RhoA proteins bound the RBD domain of the Rho  effector Rhotekin ( Fig.  8 B).	bind
30436	1	7618	5	13	NULL	NULL	NULL	HR1a/HR1b	GP		bind					RhoA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_5_2698_s_204	9446575	3 Furthermore, overlapping oligopeptides based upon RhoA covering the entire predicted binding regions for HR1a and HR1b (residues 1-100) are neither able to interact directly nor able to compete for HR1a/HR1b binding to RhoA, indicating that the sites of interaction on RhoA are sensitive to conformational constraints.	bind
23711	1	7618	6	10	NULL	0	NULL	HR1a/HR1b			bind					RhoA					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_5_2698_s_204	9446575	3 Furthermore, overlapping oligopeptides based upon RhoA covering the entire predicted binding regions for HR1a and HR1b (residues 1-100) are neither able to interact directly nor able to compete for HR1a/HR1b binding to RhoA, indicating that the sites of interaction on RhoA are sensitive to conformational constraints.	bind
46623	1	7619	5	13	NULL	NULL	NULL	genomic DNA sequences	NucleicAcid		bind					SATB1	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_17_11463_s_224	9111059	3 Genomic DNA sequences that are bound to SATB1  in vivo have recently been characterized based on cross-linking techniques.	bind
23339	1	7619	6	10	NULL	0	NULL	genomic DNA sequences	NULL		bind	NULL				SATB1	NULL				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_17_11463_s_224	9111059	3 Genomic DNA sequences that are bound to SATB1  in vivo have recently been characterized based on cross-linking techniques.	bind
30439	1	7620	5	13	NULL	NULL	NULL	Git2	GP		is homologous to		highly			p95PKL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_8_6037_s_312	11096073	3 Git2 is highly homologous to p95PKL; and we indeed detected ternary complexes of paxillin alpha/Git2/betaPIX, and Git2/betaPIX/PAK3.2 However, since paxillin alpha itself can bind to PAK3, we could not properly assess whether or not these four proteins make the tetra-protein complex in a linear configuration.	bind
30440	2	7620	5	13	NULL	NULL	NULL	paxillin alpha	GP		bind					PAK3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_8_6037_s_312	11096073	3 Git2 is highly homologous to p95PKL; and we indeed detected ternary complexes of paxillin alpha/Git2/betaPIX, and Git2/betaPIX/PAK3.2 However, since paxillin alpha itself can bind to PAK3, we could not properly assess whether or not these four proteins make the tetra-protein complex in a linear configuration.	bind
23713	1	7620	6	NULL	NULL	0	NULL	Git2	NULL		is homologous to	NULL	highly			p95PKL	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_8_6037_s_312	11096073	3 Git2 is highly homologous to p95PKL; and we indeed detected ternary complexes of paxillin alpha/Git2/betaPIX, and Git2/betaPIX/PAK3.2 However, since paxillin alpha itself can bind to PAK3, we could not properly assess whether or not these four proteins make the tetra-protein complex in a linear configuration.	bind
23714	2	7620	6	NULL	NULL	0	NULL	paxillin alpha	NULL		bind	NULL				PAK3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_8_6037_s_312	11096073	3 Git2 is highly homologous to p95PKL; and we indeed detected ternary complexes of paxillin alpha/Git2/betaPIX, and Git2/betaPIX/PAK3.2 However, since paxillin alpha itself can bind to PAK3, we could not properly assess whether or not these four proteins make the tetra-protein complex in a linear configuration.	bind
30441	1	7621	5	13	NULL	NULL	NULL	ADP	Chemical		bind					Pgp	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_45_46518_s_314	15326176	3 Given the very low turnover rate evident for mutant E552A/S528A in  Fig. 6 B the fact that ADP was bound to Pgp might seem surprising.	bind
23341	1	7621	6	NULL	NULL	0	NULL	ADP	NULL		bind	NULL				Pgp	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_45_46518_s_314	15326176	3 Given the very low turnover rate evident for mutant E552A/S528A in  Fig. 6 B the fact that ADP was bound to Pgp might seem surprising.	bind
23343	2	7621	6	10	NULL	0	NULL		NULL	mutant	exhibits	NULL		E552A/S528A		low turnover rate	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_45_46518_s_314	15326176	3 Given the very low turnover rate evident for mutant E552A/S528A in  Fig. 6 B the fact that ADP was bound to Pgp might seem surprising.	bind
30442	1	7622	5	13	NULL	NULL	NULL	bZIP protein	GP		bind									ABA-responsive elements	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_1689_s_162	11704678	3 However, bZIP protein binding to ABA-responsive elements is independent of VP1/PvAlf and dependent on ABA  in vivo ( 33,  43,  67).	bind
30443	2	7622	5	13	NULL	NULL	NULL	statement 1	Process		is independent of					VP1/PvAlf	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_1689_s_162	11704678	3 However, bZIP protein binding to ABA-responsive elements is independent of VP1/PvAlf and dependent on ABA  in vivo ( 33,  43,  67).	bind
30444	3	7622	5	13	NULL	NULL	NULL	statement 1	Process		is dependent on					ABA	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_1689_s_162	11704678	3 However, bZIP protein binding to ABA-responsive elements is independent of VP1/PvAlf and dependent on ABA  in vivo ( 33,  43,  67).	bind
23345	1	7622	6	10	NULL	0	NULL	bZIP protein			bind									ABA-responsive elements	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_1689_s_162	11704678	3 However, bZIP protein binding to ABA-responsive elements is independent of VP1/PvAlf and dependent on ABA  in vivo ( 33,  43,  67).	bind
23346	2	7622	6	NULL	NULL	0	NULL	statement 1	NULL		is independent of	NULL				VP1/PvAlf	NULL				NULL	in vivo	0	NULL	NULL	NULL	gw60_jbiolchem_277_3_1689_s_162	11704678	3 However, bZIP protein binding to ABA-responsive elements is independent of VP1/PvAlf and dependent on ABA  in vivo ( 33,  43,  67).	bind
23347	3	7622	6	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				ABA	NULL				NULL	in vivo	0	NULL	NULL	NULL	gw60_jbiolchem_277_3_1689_s_162	11704678	3 However, bZIP protein binding to ABA-responsive elements is independent of VP1/PvAlf and dependent on ABA  in vivo ( 33,  43,  67).	bind
30528	1	7623	5	13	NULL	NULL	NULL	SSB protein	GP		bind					32-mer oligonucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_39_23874_s_284	8798618	3 In addition, LexA S119A repressor did not change the binding affinity of SSB protein for a 32-mer oligonucleotide or affect the apparent site size of SSB protein tetramers bound to epsilonM13 DNA.3 Therefore, there is no experimental support for proposal two.	bind
30530	2	7623	5	13	NULL	NULL	NULL	LexA repressor	GP		does not change			S119A		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_39_23874_s_284	8798618	3 In addition, LexA S119A repressor did not change the binding affinity of SSB protein for a 32-mer oligonucleotide or affect the apparent site size of SSB protein tetramers bound to epsilonM13 DNA.3 Therefore, there is no experimental support for proposal two.	bind
30532	3	7623	5	13	NULL	NULL	NULL	SSB protein tetramers	GP		bind					epsilonM13 DNA.3	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_39_23874_s_284	8798618	3 In addition, LexA S119A repressor did not change the binding affinity of SSB protein for a 32-mer oligonucleotide or affect the apparent site size of SSB protein tetramers bound to epsilonM13 DNA.3 Therefore, there is no experimental support for proposal two.	bind
30537	4	7623	5	13	NULL	NULL	NULL	LexA repressor	GP		does not affect			S119A		statement 3	Process	apparent site size of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_39_23874_s_284	8798618	3 In addition, LexA S119A repressor did not change the binding affinity of SSB protein for a 32-mer oligonucleotide or affect the apparent site size of SSB protein tetramers bound to epsilonM13 DNA.3 Therefore, there is no experimental support for proposal two.	bind
23349	1	7623	6	NULL	NULL	0	NULL	SSB protein	NULL		bind	NULL				32-mer oligonucleotide	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_39_23874_s_284	8798618	3 In addition, LexA S119A repressor did not change the binding affinity of SSB protein for a 32-mer oligonucleotide or affect the apparent site size of SSB protein tetramers bound to epsilonM13 DNA.3 Therefore, there is no experimental support for proposal two.	bind
23350	2	7623	6	10	NULL	0	NULL	LexA repressor	NULL		does not change	NULL		S119A		statement 1	NULL	binding affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_39_23874_s_284	8798618	3 In addition, LexA S119A repressor did not change the binding affinity of SSB protein for a 32-mer oligonucleotide or affect the apparent site size of SSB protein tetramers bound to epsilonM13 DNA.3 Therefore, there is no experimental support for proposal two.	bind
23351	3	7623	6	NULL	NULL	0	NULL	SSB protein tetramers	NULL		bind	NULL				epsilonM13 DNA.3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_39_23874_s_284	8798618	3 In addition, LexA S119A repressor did not change the binding affinity of SSB protein for a 32-mer oligonucleotide or affect the apparent site size of SSB protein tetramers bound to epsilonM13 DNA.3 Therefore, there is no experimental support for proposal two.	bind
46624	4	7623	6	10	NULL	0	NULL	LexA repressor	NULL		does not change	NULL		S119A		statement 3	NULL	apparent site size of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_39_23874_s_284	8798618	3 In addition, LexA S119A repressor did not change the binding affinity of SSB protein for a 32-mer oligonucleotide or affect the apparent site size of SSB protein tetramers bound to epsilonM13 DNA.3 Therefore, there is no experimental support for proposal two.	bind
30539	1	7624	5	13	NULL	NULL	NULL	PP14	GP		bind					alpha2-macroglobulin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_16_14059_s_194	12556471	3 In addition, PP14 binds to the large serum carrier protein alpha2-macroglobulin, which potentiates the T cell inhibitory activity of PP14 ( ).	bind
30540	2	7624	5	13	NULL	NULL	NULL	alpha2-macroglobulin	GP		is a type of					large serum carrier protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_16_14059_s_194	12556471	3 In addition, PP14 binds to the large serum carrier protein alpha2-macroglobulin, which potentiates the T cell inhibitory activity of PP14 ( ).	bind
30541	4	7624	5	13	NULL	NULL	NULL	alpha2-macroglobulin	GP		potentiates					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_16_14059_s_194	12556471	3 In addition, PP14 binds to the large serum carrier protein alpha2-macroglobulin, which potentiates the T cell inhibitory activity of PP14 ( ).	bind
46625	3	7624	5	13	NULL	NULL	NULL	PP14	GP		inhibit					T cell	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_16_14059_s_194	12556471	3 In addition, PP14 binds to the large serum carrier protein alpha2-macroglobulin, which potentiates the T cell inhibitory activity of PP14 ( ).	bind
23353	1	7624	6	10	NULL	0	NULL	PP14	NULL		bind	NULL				 alpha2-macroglobulin	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_16_14059_s_194	12556471	3 In addition, PP14 binds to the large serum carrier protein alpha2-macroglobulin, which potentiates the T cell inhibitory activity of PP14 ( ).	bind
23354	2	7624	6	10	NULL	0	NULL	alpha2-macroglobulin	NULL		is a type of	NULL				large serum carrier protein	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_16_14059_s_194	12556471	3 In addition, PP14 binds to the large serum carrier protein alpha2-macroglobulin, which potentiates the T cell inhibitory activity of PP14 ( ).	bind
23356	4	7624	6	10	NULL	0	NULL	 alpha2-macroglobulin	NULL		potentiates	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_16_14059_s_194	12556471	3 In addition, PP14 binds to the large serum carrier protein alpha2-macroglobulin, which potentiates the T cell inhibitory activity of PP14 ( ).	bind
46626	3	7624	6	10	NULL	0	NULL	PP14	NULL		inhibit	NULL				T cell	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_16_14059_s_194	12556471	3 In addition, PP14 binds to the large serum carrier protein alpha2-macroglobulin, which potentiates the T cell inhibitory activity of PP14 ( ).	bind
30551	1	7626	5	13	NULL	NULL	NULL	iNOS	GP	purified	bind		high affinity			iNOS monomers	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_1_295_s_268	11689556	3 In addition, spectral binding experiments with purified iNOS confirm high affinity binding to iNOS monomers ( K s < =50 nM) but low affinity binding to iNOS dimers ( K s > 10 muM).	bind
30552	2	7626	5	13	NULL	NULL	NULL	iNOS	GP	purified	bind		low affinity			iNOS dimers	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_1_295_s_268	11689556	3 In addition, spectral binding experiments with purified iNOS confirm high affinity binding to iNOS monomers ( K s < =50 nM) but low affinity binding to iNOS dimers ( K s > 10 muM).	bind
23359	1	7626	6	NULL	NULL	0	NULL	iNOS	NULL	purified	bind	NULL	high affinity			iNOS monomers	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_1_295_s_268	11689556	3 In addition, spectral binding experiments with purified iNOS confirm high affinity binding to iNOS monomers ( K s < =50 nM) but low affinity binding to iNOS dimers ( K s > 10 muM).	bind
23360	2	7626	6	NULL	NULL	0	NULL	iNOS	NULL	purified	bind	NULL	low affinity			iNOS dimers	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_1_295_s_268	11689556	3 In addition, spectral binding experiments with purified iNOS confirm high affinity binding to iNOS monomers ( K s < =50 nM) but low affinity binding to iNOS dimers ( K s > 10 muM).	bind
30557	1	7628	5	13	NULL	NULL	NULL	PD180970	Chemical		inhibit					Src	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24935_s_337	10823829	3 Inhibition of Src or JAKs by PD180970 or AG490, respectively, results in inactivation of Stat3 DNA binding activity and growth inhibition of these breast cancer cells.	bind
30558	2	7628	5	13	NULL	NULL	NULL	AG490	Chemical		inhibit					JAK	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24935_s_337	10823829	3 Inhibition of Src or JAKs by PD180970 or AG490, respectively, results in inactivation of Stat3 DNA binding activity and growth inhibition of these breast cancer cells.	bind
30560	3	7628	5	13	NULL	NULL	NULL	Stat3	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24935_s_337	10823829	3 Inhibition of Src or JAKs by PD180970 or AG490, respectively, results in inactivation of Stat3 DNA binding activity and growth inhibition of these breast cancer cells.	bind
30561	4	7628	5	13	NULL	NULL	NULL	statement 1	Process		inactivates					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24935_s_337	10823829	3 Inhibition of Src or JAKs by PD180970 or AG490, respectively, results in inactivation of Stat3 DNA binding activity and growth inhibition of these breast cancer cells.	bind
30562	5	7628	5	13	NULL	NULL	NULL	statement 2	Process		inactivates					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24935_s_337	10823829	3 Inhibition of Src or JAKs by PD180970 or AG490, respectively, results in inactivation of Stat3 DNA binding activity and growth inhibition of these breast cancer cells.	bind
30564	6	7628	5	13	NULL	NULL	NULL	statement 1	Process		inhibits					breast cancer cells	Cell	growth of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24935_s_337	10823829	3 Inhibition of Src or JAKs by PD180970 or AG490, respectively, results in inactivation of Stat3 DNA binding activity and growth inhibition of these breast cancer cells.	bind
30565	7	7628	5	13	NULL	NULL	NULL	statement 2 	Process		inhibits					breast cancer cells	Cell	growth of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24935_s_337	10823829	3 Inhibition of Src or JAKs by PD180970 or AG490, respectively, results in inactivation of Stat3 DNA binding activity and growth inhibition of these breast cancer cells.	bind
23715	1	7628	6	NULL	NULL	0	NULL	PD180970	NULL		inhibits	NULL				Src	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24935_s_337	10823829	3 Inhibition of Src or JAKs by PD180970 or AG490, respectively, results in inactivation of Stat3 DNA binding activity and growth inhibition of these breast cancer cells.	bind
23716	2	7628	6	NULL	NULL	0	NULL	AG490	NULL		inhibit	NULL				JAK	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24935_s_337	10823829	3 Inhibition of Src or JAKs by PD180970 or AG490, respectively, results in inactivation of Stat3 DNA binding activity and growth inhibition of these breast cancer cells.	bind
23717	4	7628	6	10	NULL	0	NULL	statement 1	NULL		inactivate	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24935_s_337	10823829	3 Inhibition of Src or JAKs by PD180970 or AG490, respectively, results in inactivation of Stat3 DNA binding activity and growth inhibition of these breast cancer cells.	bind
23718	5	7628	6	10	NULL	0	NULL	statement 2	NULL		inactivate	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24935_s_337	10823829	3 Inhibition of Src or JAKs by PD180970 or AG490, respectively, results in inactivation of Stat3 DNA binding activity and growth inhibition of these breast cancer cells.	bind
46627	3	7628	6	10	NULL	0	NULL	Stat3	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24935_s_337	10823829	3 Inhibition of Src or JAKs by PD180970 or AG490, respectively, results in inactivation of Stat3 DNA binding activity and growth inhibition of these breast cancer cells.	bind
46628	6	7628	6	10	NULL	0	NULL	statement 1	NULL		inhibit	NULL				breast cancer cells	NULL	growth of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24935_s_337	10823829	3 Inhibition of Src or JAKs by PD180970 or AG490, respectively, results in inactivation of Stat3 DNA binding activity and growth inhibition of these breast cancer cells.	bind
46629	7	7628	6	10	NULL	0	NULL	statement 2	NULL		inhibit	NULL				breast cancer cells	NULL	growth of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24935_s_337	10823829	3 Inhibition of Src or JAKs by PD180970 or AG490, respectively, results in inactivation of Stat3 DNA binding activity and growth inhibition of these breast cancer cells.	bind
30578	1	7629	5	13	NULL	NULL	NULL	GTP gammaS	GP		bind		high-affinity			G alpha	GP		i3 subunits		NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_6_1077_s_8	12684263	3 Isotopic dilution experiments ([35]GTP gammaS  versus GTP gammaS) revealed high-affinity [35]GTP gammaS binding to G alphai3 subunits in the absence of receptor ligands indicating constitutive activity.	bind
30579	2	7629	5	13	NULL	NULL	NULL	statement 1	Process		in the absence of					receptor ligands	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_6_1077_s_8	12684263	3 Isotopic dilution experiments ([35]GTP gammaS  versus GTP gammaS) revealed high-affinity [35]GTP gammaS binding to G alphai3 subunits in the absence of receptor ligands indicating constitutive activity.	bind
23493	1	7629	6	10	NULL	0	NULL	GTP gammaS	NULL		bind	NULL	high affinity			G alpha	NULL		i3 subunits		NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_6_1077_s_8	12684263	3 Isotopic dilution experiments ([35]GTP gammaS  versus GTP gammaS) revealed high-affinity [35]GTP gammaS binding to G alphai3 subunits in the absence of receptor ligands indicating constitutive activity.	bind
23494	2	7629	6	NULL	NULL	0	NULL	statement 1	NULL		occurs in absence of	NULL				receptor ligands	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_138_6_1077_s_8	12684263	3 Isotopic dilution experiments ([35]GTP gammaS  versus GTP gammaS) revealed high-affinity [35]GTP gammaS binding to G alphai3 subunits in the absence of receptor ligands indicating constitutive activity.	bind
30584	1	7630	5	13	NULL	NULL	NULL	AGL15	GP		bind					DTA3	GP			regulatory regions	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_30_28154_s_271	12743119	3 It  seems likely that co-factors are involved in binding of AGL15 to  DTA3  regulatory regions  in vivo.	bind
30606	2	7630	5	13	NULL	NULL	NULL	co-factors	Chemical		involved in					statement 1	Process				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_30_28154_s_271	12743119	3 It  seems likely that co-factors are involved in binding of AGL15 to  DTA3  regulatory regions  in vivo.	bind
23555	1	7630	6	NULL	NULL	0	NULL	AGL15	NULL		bind	NULL				DTA3	NULL			regulatory region	NULL	in vivo	0	NULL	NULL	NULL	gw70_jbiolchem_278_30_28154_s_271	12743119	3 It  seems likely that co-factors are involved in binding of AGL15 to  DTA3  regulatory regions  in vivo.	bind
23556	2	7630	6	10	NULL	0	NULL	co-factors			are involved in					statement 1					NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_30_28154_s_271	12743119	3 It  seems likely that co-factors are involved in binding of AGL15 to  DTA3  regulatory regions  in vivo.	bind
30615	1	7631	5	13	NULL	NULL	NULL	Mx1	GP		bind					GTP	Chemical				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_45_32071_s_242	10542240	3 It has been previously demonstrated by  in vitro studies that the GTP binding activity of Mx1 or MxA protein is sufficient to exert antiviral activity ( 12).	bind
30616	2	7631	5	13	NULL	NULL	NULL	MxA protein	GP		bind					GTP	Chemical				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_45_32071_s_242	10542240	3 It has been previously demonstrated by  in vitro studies that the GTP binding activity of Mx1 or MxA protein is sufficient to exert antiviral activity ( 12).	bind
46630	3	7631	5	13	NULL	NULL	NULL	statement 1	Process		is sufficient for					antiviral activity	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_45_32071_s_242	10542240	3 It has been previously demonstrated by  in vitro studies that the GTP binding activity of Mx1 or MxA protein is sufficient to exert antiviral activity ( 12).	bind
46631	4	7631	5	13	NULL	NULL	NULL	statement 2	Process		is sufficient for					antiviral activity	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_45_32071_s_242	10542240	3 It has been previously demonstrated by  in vitro studies that the GTP binding activity of Mx1 or MxA protein is sufficient to exert antiviral activity ( 12).	bind
23557	1	7631	6	NULL	NULL	0	NULL	Mx1	NULL		bind	NULL				GTP	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_45_32071_s_242	10542240	3 It has been previously demonstrated by  in vitro studies that the GTP binding activity of Mx1 or MxA protein is sufficient to exert antiviral activity ( 12).	bind
23558	2	7631	6	NULL	NULL	0	NULL	MxA protein	NULL		bind	NULL				GTP	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_274_45_32071_s_242	10542240	3 It has been previously demonstrated by  in vitro studies that the GTP binding activity of Mx1 or MxA protein is sufficient to exert antiviral activity ( 12).	bind
23559	3	7631	6	10	NULL	0	NULL	statement 1			is sufficient for					antiviral activity					NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_45_32071_s_242	10542240	3 It has been previously demonstrated by  in vitro studies that the GTP binding activity of Mx1 or MxA protein is sufficient to exert antiviral activity ( 12).	bind
23560	4	7631	6	10	NULL	0	NULL	statement 2			is sufficient for					antiviral activity					NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_45_32071_s_242	10542240	3 It has been previously demonstrated by  in vitro studies that the GTP binding activity of Mx1 or MxA protein is sufficient to exert antiviral activity ( 12).	bind
30625	1	7632	5	13	NULL	NULL	NULL	1-(bromomethyl)phenanthrene	Chemical		does not bind		efficiently			AAC(6'')-Ii	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_15_12873_s_206	12566434	3 Its inability to inactivate AAC(6'')-Ii could be because 1-(bromomethyl)phenanthrene can not efficiently bind to AAC(6'')-Ii or because AAC(6'')-Ii lacks an appropriate active site residue to serve as the nucleophile in the reaction.	bind
30626	2	7632	5	13	NULL	NULL	NULL	AAC(6'')-Ii	GP		lacks								active site residue		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_15_12873_s_206	12566434	3 Its inability to inactivate AAC(6'')-Ii could be because 1-(bromomethyl)phenanthrene can not efficiently bind to AAC(6'')-Ii or because AAC(6'')-Ii lacks an appropriate active site residue to serve as the nucleophile in the reaction.	bind
30628	3	7632	5	13	NULL	NULL	NULL	AAC(6'')-Ii	GP		serve as			active site residue		nucleophile	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_15_12873_s_206	12566434	3 Its inability to inactivate AAC(6'')-Ii could be because 1-(bromomethyl)phenanthrene can not efficiently bind to AAC(6'')-Ii or because AAC(6'')-Ii lacks an appropriate active site residue to serve as the nucleophile in the reaction.	bind
23561	1	7632	6	10	NULL	0	NULL	1-(bromomethyl)phenanthrene	NULL		does not bind	NULL	efficiently			AAC(6'')-Ii	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_15_12873_s_206	12566434	3 Its inability to inactivate AAC(6'')-Ii could be because 1-(bromomethyl)phenanthrene can not efficiently bind to AAC(6'')-Ii or because AAC(6'')-Ii lacks an appropriate active site residue to serve as the nucleophile in the reaction.	bind
23562	2	7632	6	10	NULL	0	NULL	AAC(6'')-Ii	NULL		lacks	NULL					NULL		active site residue		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_15_12873_s_206	12566434	3 Its inability to inactivate AAC(6'')-Ii could be because 1-(bromomethyl)phenanthrene can not efficiently bind to AAC(6'')-Ii or because AAC(6'')-Ii lacks an appropriate active site residue to serve as the nucleophile in the reaction.	bind
55530	3	7632	6	10	NULL	0	NULL	AAC(6'')-Ii			serves as			active site residue		nucleophile					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_15_12873_s_206	12566434	3 Its inability to inactivate AAC(6'')-Ii could be because 1-(bromomethyl)phenanthrene can not efficiently bind to AAC(6'')-Ii or because AAC(6'')-Ii lacks an appropriate active site residue to serve as the nucleophile in the reaction.	bind
30641	1	7633	5	13	NULL	NULL	NULL	gankyrin	GP		bind					Rb	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_12_10668_s_229	12525503	3 MAGE-A4 did not reduce the binding of gankyrin to Rb, S6, or Cdk4.	bind
30642	2	7633	5	13	NULL	NULL	NULL	gankyrin	GP		bind					S6	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_12_10668_s_229	12525503	3 MAGE-A4 did not reduce the binding of gankyrin to Rb, S6, or Cdk4.	bind
30643	3	7633	5	13	NULL	NULL	NULL	gankyrin	GP		bind					Cdk4	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_12_10668_s_229	12525503	3 MAGE-A4 did not reduce the binding of gankyrin to Rb, S6, or Cdk4.	bind
30645	4	7633	5	13	NULL	NULL	NULL	statement 1	Process		is alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_12_10668_s_229	12525503	3 MAGE-A4 did not reduce the binding of gankyrin to Rb, S6, or Cdk4.	bind
30646	5	7633	5	13	NULL	NULL	NULL	statement 1	Process		is alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_12_10668_s_229	12525503	3 MAGE-A4 did not reduce the binding of gankyrin to Rb, S6, or Cdk4.	bind
30648	6	7633	5	13	NULL	NULL	NULL	MAGE-A4	GP		does not reduce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_12_10668_s_229	12525503	3 MAGE-A4 did not reduce the binding of gankyrin to Rb, S6, or Cdk4.	bind
30651	7	7633	5	13	NULL	NULL	NULL	MAGE-A4	GP		does not reduce					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_12_10668_s_229	12525503	3 MAGE-A4 did not reduce the binding of gankyrin to Rb, S6, or Cdk4.	bind
30653	8	7633	5	13	NULL	NULL	NULL	MAGE-A4	GP		does not reduce					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_12_10668_s_229	12525503	3 MAGE-A4 did not reduce the binding of gankyrin to Rb, S6, or Cdk4.	bind
23563	1	7633	6	NULL	NULL	0	NULL	gankyrin	NULL		bind	NULL				Rb	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10668_s_229	12525503	3 MAGE-A4 did not reduce the binding of gankyrin to Rb, S6, or Cdk4.	bind
23564	2	7633	6	NULL	NULL	0	NULL	gankyrin	NULL		bind	NULL				S6	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10668_s_229	12525503	3 MAGE-A4 did not reduce the binding of gankyrin to Rb, S6, or Cdk4.	bind
23565	3	7633	6	NULL	NULL	0	NULL	gankyrin	NULL		bind	NULL				Cdk4	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10668_s_229	12525503	3 MAGE-A4 did not reduce the binding of gankyrin to Rb, S6, or Cdk4.	bind
23566	4	7633	6	NULL	NULL	0	NULL	MAGE-A4	NULL		did not reduce	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10668_s_229	12525503	3 MAGE-A4 did not reduce the binding of gankyrin to Rb, S6, or Cdk4.	bind
23567	5	7633	6	NULL	NULL	0	NULL	MAGE-A4	NULL		did not reduce	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10668_s_229	12525503	3 MAGE-A4 did not reduce the binding of gankyrin to Rb, S6, or Cdk4.	bind
23568	6	7633	6	NULL	NULL	0	NULL	MAGE-A4	NULL		did not reduce	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10668_s_229	12525503	3 MAGE-A4 did not reduce the binding of gankyrin to Rb, S6, or Cdk4.	bind
46632	7	7633	6	10	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10668_s_229	12525503	3 MAGE-A4 did not reduce the binding of gankyrin to Rb, S6, or Cdk4.	bind
46633	8	7633	6	10	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10668_s_229	12525503	3 MAGE-A4 did not reduce the binding of gankyrin to Rb, S6, or Cdk4.	bind
30693	1	7634	5	13	NULL	NULL	NULL	karyopherin beta	GP		bind					C-Nup1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_31_19538_s_91	9235958	3 Most importantly, when karyopherin alpha and RanGAP were added together, karyopherin beta binding to C-Nup1 was restored ( lane 5).	bind
30694	2	7634	5	13	NULL	NULL	NULL	karyopherin alpha 	GP		is added together with					RanGAP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_31_19538_s_91	9235958	3 Most importantly, when karyopherin alpha and RanGAP were added together, karyopherin beta binding to C-Nup1 was restored ( lane 5).	bind
46634	3	7634	5	13	NULL	NULL	NULL	statement 2	Process		restores					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_31_19538_s_91	9235958	3 Most importantly, when karyopherin alpha and RanGAP were added together, karyopherin beta binding to C-Nup1 was restored ( lane 5).	bind
23569	1	7634	6	NULL	NULL	0	NULL	karyopherin beta	NULL		bind	NULL				C-Nup1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_31_19538_s_91	9235958	3 Most importantly, when karyopherin alpha and RanGAP were added together, karyopherin beta binding to C-Nup1 was restored ( lane 5).	bind
23570	2	7634	6	NULL	NULL	0	NULL	karyopherin alpha	NULL		is added together with	NULL				RanGAP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_31_19538_s_91	9235958	3 Most importantly, when karyopherin alpha and RanGAP were added together, karyopherin beta binding to C-Nup1 was restored ( lane 5).	bind
23571	3	7634	6	NULL	NULL	0	NULL	statement 2	NULL		restores	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_31_19538_s_91	9235958	3 Most importantly, when karyopherin alpha and RanGAP were added together, karyopherin beta binding to C-Nup1 was restored ( lane 5).	bind
30697	1	7639	5	13	NULL	NULL	NULL	ISP	GP		bind					complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_13_12951_s_272	14718526	3 Mutation to aspartate may increase the stability of binding of the ISP to the complex.	bind
30698	2	7639	5	13	NULL	NULL	NULL	aspartate	Chemical	mutation to	increase		may			statement 1	Process	stability of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_13_12951_s_272	14718526	3 Mutation to aspartate may increase the stability of binding of the ISP to the complex.	bind
23572	1	7639	6	NULL	NULL	0	NULL	ISP	NULL		bind	NULL				complex	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12951_s_272	14718526	3 Mutation to aspartate may increase the stability of binding of the ISP to the complex.	bind
23573	2	7639	6	NULL	NULL	0	NULL	aspartate	NULL	mutant	increase	NULL	may			statement 1	NULL	stability of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12951_s_272	14718526	3 Mutation to aspartate may increase the stability of binding of the ISP to the complex.	bind
30832	2	7641	5	13	NULL	NULL	NULL	F-actin	GP		does not mediate					alpha-actinin	GP	recruitment of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_19_13410_s_281	10224105	3 Nevertheless, in the case of zyxin, we can rule out the possibility that alpha-actinin recruitment is primarily due to an indirect association mediated by F-actin ( 18) or some other protein(s): a deletion, which is confined to a short zyxin peptide motif that has been positively identified as an alpha-actinin binding site in a parallel  in vitro assay, virtually abolishes alpha-actinin recruitment in the targeting assay and alpha-actinin binding to GST-zyxin fusion proteins in blot overlays  in vitro.	bind
30833	3	7641	5	13	NULL	NULL	NULL	zyxin peptide	GP		is identified as			short motif					alpha-actinin binding site		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_19_13410_s_281	10224105	3 Nevertheless, in the case of zyxin, we can rule out the possibility that alpha-actinin recruitment is primarily due to an indirect association mediated by F-actin ( 18) or some other protein(s): a deletion, which is confined to a short zyxin peptide motif that has been positively identified as an alpha-actinin binding site in a parallel  in vitro assay, virtually abolishes alpha-actinin recruitment in the targeting assay and alpha-actinin binding to GST-zyxin fusion proteins in blot overlays  in vitro.	bind
32235	4	7641	5	13	NULL	NULL	NULL	statement 3	GP	deletion of	abolishes					alpha-actinin	GP	recruitment of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_19_13410_s_281	10224105	3 Nevertheless, in the case of zyxin, we can rule out the possibility that alpha-actinin recruitment is primarily due to an indirect association mediated by F-actin ( 18) or some other protein(s): a deletion, which is confined to a short zyxin peptide motif that has been positively identified as an alpha-actinin binding site in a parallel  in vitro assay, virtually abolishes alpha-actinin recruitment in the targeting assay and alpha-actinin binding to GST-zyxin fusion proteins in blot overlays  in vitro.	bind
32236	5	7641	5	13	NULL	NULL	NULL	alpha-actinin	GP		bind					GST-zyxin fusion proteins	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_19_13410_s_281	10224105	3 Nevertheless, in the case of zyxin, we can rule out the possibility that alpha-actinin recruitment is primarily due to an indirect association mediated by F-actin ( 18) or some other protein(s): a deletion, which is confined to a short zyxin peptide motif that has been positively identified as an alpha-actinin binding site in a parallel  in vitro assay, virtually abolishes alpha-actinin recruitment in the targeting assay and alpha-actinin binding to GST-zyxin fusion proteins in blot overlays  in vitro.	bind
32237	6	7641	5	13	NULL	NULL	NULL	statement 3	GP	deletion of	abolishes					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_19_13410_s_281	10224105	3 Nevertheless, in the case of zyxin, we can rule out the possibility that alpha-actinin recruitment is primarily due to an indirect association mediated by F-actin ( 18) or some other protein(s): a deletion, which is confined to a short zyxin peptide motif that has been positively identified as an alpha-actinin binding site in a parallel  in vitro assay, virtually abolishes alpha-actinin recruitment in the targeting assay and alpha-actinin binding to GST-zyxin fusion proteins in blot overlays  in vitro.	bind
23781	1	7641	6	NULL	NULL	0	NULL	alpha-actinin	NULL		bind	NULL				GST-zyxin fusion protein	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_274_19_13410_s_281	10224105	3 Nevertheless, in the case of zyxin, we can rule out the possibility that alpha-actinin recruitment is primarily due to an indirect association mediated by F-actin ( 18) or some other protein(s): a deletion, which is confined to a short zyxin peptide motif that has been positively identified as an alpha-actinin binding site in a parallel  in vitro assay, virtually abolishes alpha-actinin recruitment in the targeting assay and alpha-actinin binding to GST-zyxin fusion proteins in blot overlays  in vitro.	bind
46888	2	7641	6	NULL	NULL	0	NULL	zyxin peptide motif	NULL	deletion of	abolishes	NULL				alpha-actinin	NULL	recruitment of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_19_13410_s_281	10224105	3 Nevertheless, in the case of zyxin, we can rule out the possibility that alpha-actinin recruitment is primarily due to an indirect association mediated by F-actin ( 18) or some other protein(s): a deletion, which is confined to a short zyxin peptide motif that has been positively identified as an alpha-actinin binding site in a parallel  in vitro assay, virtually abolishes alpha-actinin recruitment in the targeting assay and alpha-actinin binding to GST-zyxin fusion proteins in blot overlays  in vitro.	bind
46889	3	7641	6	NULL	NULL	0	NULL	zyxin peptide motif	NULL	deletion of	abolishes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_19_13410_s_281	10224105	3 Nevertheless, in the case of zyxin, we can rule out the possibility that alpha-actinin recruitment is primarily due to an indirect association mediated by F-actin ( 18) or some other protein(s): a deletion, which is confined to a short zyxin peptide motif that has been positively identified as an alpha-actinin binding site in a parallel  in vitro assay, virtually abolishes alpha-actinin recruitment in the targeting assay and alpha-actinin binding to GST-zyxin fusion proteins in blot overlays  in vitro.	bind
30699	1	7642	5	13	NULL	NULL	NULL	dN-Occ	GP		bind		nonspecific			protein A/G-IgG	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49644_s_277	14512431	3 Nonspecific binding of dN-Occ to protein A/G-IgG (GFAP antibody) did occur at a level of about 50% of the maximal specific binding, but was not concentration-dependent.	bind
30700	2	7642	5	13	NULL	NULL	NULL	protein A/G-IgG	GP		is a type of					GFAP antibody	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49644_s_277	14512431	3 Nonspecific binding of dN-Occ to protein A/G-IgG (GFAP antibody) did occur at a level of about 50% of the maximal specific binding, but was not concentration-dependent.	bind
30701	3	7642	5	13	NULL	NULL	NULL	statement 1	Process		is not dependent on					concentration					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49644_s_277	14512431	3 Nonspecific binding of dN-Occ to protein A/G-IgG (GFAP antibody) did occur at a level of about 50% of the maximal specific binding, but was not concentration-dependent.	bind
23574	1	7642	6	NULL	NULL	0	NULL	dN-Occ	NULL		bind	NULL	non-specifically			protein A/G-IgG	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49644_s_277	14512431	3 Nonspecific binding of dN-Occ to protein A/G-IgG (GFAP antibody) did occur at a level of about 50% of the maximal specific binding, but was not concentration-dependent.	bind
23575	2	7642	6	NULL	NULL	0	NULL	statement 1	NULL		is not dependent on	NULL				concentration	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49644_s_277	14512431	3 Nonspecific binding of dN-Occ to protein A/G-IgG (GFAP antibody) did occur at a level of about 50% of the maximal specific binding, but was not concentration-dependent.	bind
46635	3	7642	6	10	NULL	0	NULL	protein A/G-IgG	NULL		is a type of	NULL				GFAP antibody	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49644_s_277	14512431	3 Nonspecific binding of dN-Occ to protein A/G-IgG (GFAP antibody) did occur at a level of about 50% of the maximal specific binding, but was not concentration-dependent.	bind
30702	1	7643	5	13	NULL	NULL	NULL	ATP	Chemical		bind					ORC-5A	GP		Orc5p		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_185	12966094	3 One possible explanation is that in ORC-5A, the lack of ATP binding to Orc5p inhibits the ATP binding to Orc1p, thus inhibiting the ORC binding to origin DNA and leaving the entire complex sensitive to protein degradation.	bind
30703	2	7643	5	13	NULL	NULL	NULL	ATP	Chemical		bind					ORC-5A	GP		Orc1p		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_185	12966094	3 One possible explanation is that in ORC-5A, the lack of ATP binding to Orc5p inhibits the ATP binding to Orc1p, thus inhibiting the ORC binding to origin DNA and leaving the entire complex sensitive to protein degradation.	bind
30704	3	7643	5	13	NULL	NULL	NULL	statement 1	Process	lack of	inhibits					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_185	12966094	3 One possible explanation is that in ORC-5A, the lack of ATP binding to Orc5p inhibits the ATP binding to Orc1p, thus inhibiting the ORC binding to origin DNA and leaving the entire complex sensitive to protein degradation.	bind
30705	4	7643	5	13	NULL	NULL	NULL	ORC	GP		bind					origin DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_185	12966094	3 One possible explanation is that in ORC-5A, the lack of ATP binding to Orc5p inhibits the ATP binding to Orc1p, thus inhibiting the ORC binding to origin DNA and leaving the entire complex sensitive to protein degradation.	bind
30706	5	7643	5	13	NULL	NULL	NULL	statement 3	Process		inhibits					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_185	12966094	3 One possible explanation is that in ORC-5A, the lack of ATP binding to Orc5p inhibits the ATP binding to Orc1p, thus inhibiting the ORC binding to origin DNA and leaving the entire complex sensitive to protein degradation.	bind
30707	6	7643	5	13	NULL	NULL	NULL	statement 1	Process		is sensitive to					protein degradation	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_185	12966094	3 One possible explanation is that in ORC-5A, the lack of ATP binding to Orc5p inhibits the ATP binding to Orc1p, thus inhibiting the ORC binding to origin DNA and leaving the entire complex sensitive to protein degradation.	bind
30708	7	7643	5	13	NULL	NULL	NULL	statement 2	Process		is sensitive to					protein degradation	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_185	12966094	3 One possible explanation is that in ORC-5A, the lack of ATP binding to Orc5p inhibits the ATP binding to Orc1p, thus inhibiting the ORC binding to origin DNA and leaving the entire complex sensitive to protein degradation.	bind
30709	8	7643	5	13	NULL	NULL	NULL	statement 5	Process		leads to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_185	12966094	3 One possible explanation is that in ORC-5A, the lack of ATP binding to Orc5p inhibits the ATP binding to Orc1p, thus inhibiting the ORC binding to origin DNA and leaving the entire complex sensitive to protein degradation.	bind
30710	9	7643	5	13	NULL	NULL	NULL	statement 5	Process		leads to					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_185	12966094	3 One possible explanation is that in ORC-5A, the lack of ATP binding to Orc5p inhibits the ATP binding to Orc1p, thus inhibiting the ORC binding to origin DNA and leaving the entire complex sensitive to protein degradation.	bind
23576	1	7643	6	10	NULL	0	NULL	ATP			bind					ORC-5A			Orc5p		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_185	12966094	3 One possible explanation is that in ORC-5A, the lack of ATP binding to Orc5p inhibits the ATP binding to Orc1p, thus inhibiting the ORC binding to origin DNA and leaving the entire complex sensitive to protein degradation.	bind
23577	2	7643	6	10	NULL	0	NULL	ATP			bind					ORC-5A			Orc1p		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_185	12966094	3 One possible explanation is that in ORC-5A, the lack of ATP binding to Orc5p inhibits the ATP binding to Orc1p, thus inhibiting the ORC binding to origin DNA and leaving the entire complex sensitive to protein degradation.	bind
23578	3	7643	6	NULL	NULL	0	NULL	ORC	NULL		bind	NULL				origin DNA	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_185	12966094	3 One possible explanation is that in ORC-5A, the lack of ATP binding to Orc5p inhibits the ATP binding to Orc1p, thus inhibiting the ORC binding to origin DNA and leaving the entire complex sensitive to protein degradation.	bind
23579	4	7643	6	NULL	NULL	0	NULL	statement 1	NULL	lack of	inhibits	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_185	12966094	3 One possible explanation is that in ORC-5A, the lack of ATP binding to Orc5p inhibits the ATP binding to Orc1p, thus inhibiting the ORC binding to origin DNA and leaving the entire complex sensitive to protein degradation.	bind
23580	5	7643	6	NULL	NULL	0	NULL	statement 4	NULL		inhibits	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_185	12966094	3 One possible explanation is that in ORC-5A, the lack of ATP binding to Orc5p inhibits the ATP binding to Orc1p, thus inhibiting the ORC binding to origin DNA and leaving the entire complex sensitive to protein degradation.	bind
23581	6	7643	6	10	NULL	0	NULL	statement 1			is sensitive to					protein degradation					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_185	12966094	3 One possible explanation is that in ORC-5A, the lack of ATP binding to Orc5p inhibits the ATP binding to Orc1p, thus inhibiting the ORC binding to origin DNA and leaving the entire complex sensitive to protein degradation.	bind
55531	7	7643	6	10	NULL	0	NULL	statement 2			is sensitive to					protein degradation					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_185	12966094	3 One possible explanation is that in ORC-5A, the lack of ATP binding to Orc5p inhibits the ATP binding to Orc1p, thus inhibiting the ORC binding to origin DNA and leaving the entire complex sensitive to protein degradation.	bind
55532	8	7643	6	10	NULL	0	NULL	statement 5			leads to					statement 6					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_185	12966094	3 One possible explanation is that in ORC-5A, the lack of ATP binding to Orc5p inhibits the ATP binding to Orc1p, thus inhibiting the ORC binding to origin DNA and leaving the entire complex sensitive to protein degradation.	bind
55533	9	7643	6	10	NULL	0	NULL	statement 6			leads to					statement 7					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46440_s_185	12966094	3 One possible explanation is that in ORC-5A, the lack of ATP binding to Orc5p inhibits the ATP binding to Orc1p, thus inhibiting the ORC binding to origin DNA and leaving the entire complex sensitive to protein degradation.	bind
30712	1	7644	5	13	NULL	NULL	NULL	TIM10 complex	GP		function as					chaperone	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_39_36100_s_323	12138093	3 Our working hypothesis for the role of the 70-kDa TIM10 complex in this mechanism is that (i) it functions purely as a chaperone protecting AAC from aggregation; (ii) it remains stable as a heterohexamer; and (iii) passage of AAC onto the TIM22 complex for proper insertion is mediated by direct binding of AAC to the TIM22 complex accompanied by allosteric release of AAC from the TIM10 complex.	bind
30713	2	7644	5	13	NULL	NULL	NULL	statement 1	Process		protects					AAC	GP	aggregation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_39_36100_s_323	12138093	3 Our working hypothesis for the role of the 70-kDa TIM10 complex in this mechanism is that (i) it functions purely as a chaperone protecting AAC from aggregation; (ii) it remains stable as a heterohexamer; and (iii) passage of AAC onto the TIM22 complex for proper insertion is mediated by direct binding of AAC to the TIM22 complex accompanied by allosteric release of AAC from the TIM10 complex.	bind
30715	3	7644	5	13	NULL	NULL	NULL	TIM10 complex heterohexamer	GP		remains					stable					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_39_36100_s_323	12138093	3 Our working hypothesis for the role of the 70-kDa TIM10 complex in this mechanism is that (i) it functions purely as a chaperone protecting AAC from aggregation; (ii) it remains stable as a heterohexamer; and (iii) passage of AAC onto the TIM22 complex for proper insertion is mediated by direct binding of AAC to the TIM22 complex accompanied by allosteric release of AAC from the TIM10 complex.	bind
30716	4	7644	5	13	NULL	NULL	NULL	AAC	GP		bind		directly			TIM22 complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_39_36100_s_323	12138093	3 Our working hypothesis for the role of the 70-kDa TIM10 complex in this mechanism is that (i) it functions purely as a chaperone protecting AAC from aggregation; (ii) it remains stable as a heterohexamer; and (iii) passage of AAC onto the TIM22 complex for proper insertion is mediated by direct binding of AAC to the TIM22 complex accompanied by allosteric release of AAC from the TIM10 complex.	bind
30717	5	7644	5	13	NULL	NULL	NULL	AAC	GP		is released from		allosterically			TIM10 complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_39_36100_s_323	12138093	3 Our working hypothesis for the role of the 70-kDa TIM10 complex in this mechanism is that (i) it functions purely as a chaperone protecting AAC from aggregation; (ii) it remains stable as a heterohexamer; and (iii) passage of AAC onto the TIM22 complex for proper insertion is mediated by direct binding of AAC to the TIM22 complex accompanied by allosteric release of AAC from the TIM10 complex.	bind
30718	6	7644	5	13	NULL	NULL	NULL	statement 4	Process		is accompanied by					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_39_36100_s_323	12138093	3 Our working hypothesis for the role of the 70-kDa TIM10 complex in this mechanism is that (i) it functions purely as a chaperone protecting AAC from aggregation; (ii) it remains stable as a heterohexamer; and (iii) passage of AAC onto the TIM22 complex for proper insertion is mediated by direct binding of AAC to the TIM22 complex accompanied by allosteric release of AAC from the TIM10 complex.	bind
30719	7	7644	5	13	NULL	NULL	NULL	AAC	GP		is passed onto					TIM22 complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_39_36100_s_323	12138093	3 Our working hypothesis for the role of the 70-kDa TIM10 complex in this mechanism is that (i) it functions purely as a chaperone protecting AAC from aggregation; (ii) it remains stable as a heterohexamer; and (iii) passage of AAC onto the TIM22 complex for proper insertion is mediated by direct binding of AAC to the TIM22 complex accompanied by allosteric release of AAC from the TIM10 complex.	bind
30722	8	7644	5	13	NULL	NULL	NULL	statement 6	Process		mediate					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_39_36100_s_323	12138093	3 Our working hypothesis for the role of the 70-kDa TIM10 complex in this mechanism is that (i) it functions purely as a chaperone protecting AAC from aggregation; (ii) it remains stable as a heterohexamer; and (iii) passage of AAC onto the TIM22 complex for proper insertion is mediated by direct binding of AAC to the TIM22 complex accompanied by allosteric release of AAC from the TIM10 complex.	bind
23782	1	7644	6	NULL	NULL	0	NULL	TIM10 complex	NULL		functions as 	NULL				chaperone	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_39_36100_s_323	12138093	3 Our working hypothesis for the role of the 70-kDa TIM10 complex in this mechanism is that (i) it functions purely as a chaperone protecting AAC from aggregation; (ii) it remains stable as a heterohexamer; and (iii) passage of AAC onto the TIM22 complex for proper insertion is mediated by direct binding of AAC to the TIM22 complex accompanied by allosteric release of AAC from the TIM10 complex.	bind
23783	2	7644	6	NULL	NULL	0	NULL	statement 1	NULL		protects	NULL				AAC	NULL	aggregation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_39_36100_s_323	12138093	3 Our working hypothesis for the role of the 70-kDa TIM10 complex in this mechanism is that (i) it functions purely as a chaperone protecting AAC from aggregation; (ii) it remains stable as a heterohexamer; and (iii) passage of AAC onto the TIM22 complex for proper insertion is mediated by direct binding of AAC to the TIM22 complex accompanied by allosteric release of AAC from the TIM10 complex.	bind
23784	3	7644	6	NULL	NULL	0	NULL	TIM10 complex	NULL		remains stable as a 	NULL				heterohexamer	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_39_36100_s_323	12138093	3 Our working hypothesis for the role of the 70-kDa TIM10 complex in this mechanism is that (i) it functions purely as a chaperone protecting AAC from aggregation; (ii) it remains stable as a heterohexamer; and (iii) passage of AAC onto the TIM22 complex for proper insertion is mediated by direct binding of AAC to the TIM22 complex accompanied by allosteric release of AAC from the TIM10 complex.	bind
23785	4	7644	6	NULL	NULL	0	NULL	AAC	NULL		bind	NULL	directly			TIM22 complex	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_39_36100_s_323	12138093	3 Our working hypothesis for the role of the 70-kDa TIM10 complex in this mechanism is that (i) it functions purely as a chaperone protecting AAC from aggregation; (ii) it remains stable as a heterohexamer; and (iii) passage of AAC onto the TIM22 complex for proper insertion is mediated by direct binding of AAC to the TIM22 complex accompanied by allosteric release of AAC from the TIM10 complex.	bind
23786	5	7644	6	NULL	NULL	0	NULL	AAC	NULL		moves to	NULL				TIM22 complex	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_39_36100_s_323	12138093	3 Our working hypothesis for the role of the 70-kDa TIM10 complex in this mechanism is that (i) it functions purely as a chaperone protecting AAC from aggregation; (ii) it remains stable as a heterohexamer; and (iii) passage of AAC onto the TIM22 complex for proper insertion is mediated by direct binding of AAC to the TIM22 complex accompanied by allosteric release of AAC from the TIM10 complex.	bind
23787	6	7644	6	NULL	NULL	0	NULL	statement 5	NULL		is mediated by	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_39_36100_s_323	12138093	3 Our working hypothesis for the role of the 70-kDa TIM10 complex in this mechanism is that (i) it functions purely as a chaperone protecting AAC from aggregation; (ii) it remains stable as a heterohexamer; and (iii) passage of AAC onto the TIM22 complex for proper insertion is mediated by direct binding of AAC to the TIM22 complex accompanied by allosteric release of AAC from the TIM10 complex.	bind
23788	7	7644	6	10	NULL	0	NULL	AAC	NULL		released from	NULL	allosterically			TIM10 complex	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_39_36100_s_323	12138093	3 Our working hypothesis for the role of the 70-kDa TIM10 complex in this mechanism is that (i) it functions purely as a chaperone protecting AAC from aggregation; (ii) it remains stable as a heterohexamer; and (iii) passage of AAC onto the TIM22 complex for proper insertion is mediated by direct binding of AAC to the TIM22 complex accompanied by allosteric release of AAC from the TIM10 complex.	bind
23789	8	7644	6	NULL	NULL	0	NULL	statement 4	NULL		is accompanied by	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_39_36100_s_323	12138093	3 Our working hypothesis for the role of the 70-kDa TIM10 complex in this mechanism is that (i) it functions purely as a chaperone protecting AAC from aggregation; (ii) it remains stable as a heterohexamer; and (iii) passage of AAC onto the TIM22 complex for proper insertion is mediated by direct binding of AAC to the TIM22 complex accompanied by allosteric release of AAC from the TIM10 complex.	bind
30723	1	7645	5	13	NULL	NULL	NULL	PDX-1	GP		bind									A1 elements	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_18_11986_s_133	9115263	3 PDX-1 Is the Predominant beta Cell Activity Binding to the A1 and A2 Elements	bind
30724	2	7645	5	13	NULL	NULL	NULL	PDX-1	GP		bind									A2 elements	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_18_11986_s_133	9115263	3 PDX-1 Is the Predominant beta Cell Activity Binding to the A1 and A2 Elements	bind
46636	3	7645	5	13	NULL	NULL	NULL	PDX-1	GP		exhibit					beta cell activity	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_18_11986_s_133	9115263	3 PDX-1 Is the Predominant beta Cell Activity Binding to the A1 and A2 Elements	bind
23582	1	7645	6	NULL	NULL	0	NULL	PDX-1	NULL		bind	NULL					NULL			A1 element	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_18_11986_s_133	9115263	3 PDX-1 Is the Predominant beta Cell Activity Binding to the A1 and A2 Elements	bind
23583	2	7645	6	NULL	NULL	0	NULL	PDX-1	NULL		bind	NULL					NULL			A2 element	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_18_11986_s_133	9115263	3 PDX-1 Is the Predominant beta Cell Activity Binding to the A1 and A2 Elements	bind
23584	3	7645	6	NULL	NULL	0	NULL	PDX-1	NULL		exhibits	NULL				beta cell activity	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_18_11986_s_133	9115263	3 PDX-1 Is the Predominant beta Cell Activity Binding to the A1 and A2 Elements	bind
30729	1	7647	5	13	NULL	NULL	NULL	Sp1	GP		bind					MDR1	GP			GC element within promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_4_2979_s_142	10644769	3 Previous studies have shown that Sp1 binds to a GC element within the MDR1 promoter and is required for basal expression in a number of cell lines ( 28,  29,  49).	bind
30730	2	7647	5	13	NULL	NULL	NULL	Sp1	GP		is required for					basal expression	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_4_2979_s_142	10644769	3 Previous studies have shown that Sp1 binds to a GC element within the MDR1 promoter and is required for basal expression in a number of cell lines ( 28,  29,  49).	bind
23585	1	7647	6	NULL	NULL	0	NULL	Sp1	NULL		bind	NULL				MDR1	NULL			GC element of the promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_4_2979_s_142	10644769	3 Previous studies have shown that Sp1 binds to a GC element within the MDR1 promoter and is required for basal expression in a number of cell lines ( 28,  29,  49).	bind
23586	2	7647	6	NULL	NULL	0	NULL	Sp1	NULL		is required for	NULL				basal expression	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_4_2979_s_142	10644769	3 Previous studies have shown that Sp1 binds to a GC element within the MDR1 promoter and is required for basal expression in a number of cell lines ( 28,  29,  49).	bind
30733	1	7648	5	13	NULL	NULL	NULL	AMP	Chemical		bind					GS	GP	E. coli			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_39_33298_s_180	16055443	3 Previous studies on the binding of AMP to  E. coli GS found a binding constant of 125 muM and a stoichiometry of 1 mol of AMP/mol of subunit ( ).	bind
23587	1	7648	6	NULL	NULL	0	NULL	AMP	NULL		bind	NULL				GS	NULL	E.coli			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_39_33298_s_180	16055443	3 Previous studies on the binding of AMP to  E. coli GS found a binding constant of 125 muM and a stoichiometry of 1 mol of AMP/mol of subunit ( ).	bind
30731	1	7649	5	13	NULL	NULL	NULL	Rad24p protein	GP		bind					Cdc25p	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_20_5483_s_231	11032815	3 protein Rad24p binds to Cdc25p after Chk1 phosphorylation ( Lopez-Girona   et al., 1999).	bind
30732	2	7649	5	13	NULL	NULL	NULL	statement 1	Process		occurs after					Chk1	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_20_5483_s_231	11032815	3 protein Rad24p binds to Cdc25p after Chk1 phosphorylation ( Lopez-Girona   et al., 1999).	bind
23588	1	7649	6	NULL	NULL	0	NULL	Rad24p protein	NULL		bind	NULL				Cdc25p	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_19_20_5483_s_231	11032815	3 protein Rad24p binds to Cdc25p after Chk1 phosphorylation ( Lopez-Girona   et al., 1999).	bind
23589	2	7649	6	NULL	NULL	0	NULL	statement 1	NULL		occurs after	NULL				Chk1	NULL	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_embo_19_20_5483_s_231	11032815	3 protein Rad24p binds to Cdc25p after Chk1 phosphorylation ( Lopez-Girona   et al., 1999).	bind
30734	1	7651	5	13	NULL	NULL	NULL	tapasin	GP		bind			interchain disulfide bond		ERp57	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_47_44838_s_226	12239218	3 Recently it has been shown that tapasin binds to ERp57 via an interchain disulfide bond, and cooperates with ERp57 in forming the correct disulfide bonds in the class I heavy chain ( 49).	bind
30735	2	7651	5	13	NULL	NULL	NULL	ERp57	GP		forms					disulfide bonds	GP	correct			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_47_44838_s_226	12239218	3 Recently it has been shown that tapasin binds to ERp57 via an interchain disulfide bond, and cooperates with ERp57 in forming the correct disulfide bonds in the class I heavy chain ( 49).	bind
30736	3	7651	5	13	NULL	NULL	NULL	statement 2	Process		occurs in					class I heavy chain	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_47_44838_s_226	12239218	3 Recently it has been shown that tapasin binds to ERp57 via an interchain disulfide bond, and cooperates with ERp57 in forming the correct disulfide bonds in the class I heavy chain ( 49).	bind
30737	4	7651	5	13	NULL	NULL	NULL	tapasin	GP		cooperates with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_47_44838_s_226	12239218	3 Recently it has been shown that tapasin binds to ERp57 via an interchain disulfide bond, and cooperates with ERp57 in forming the correct disulfide bonds in the class I heavy chain ( 49).	bind
23590	1	7651	6	NULL	NULL	0	NULL	tapasin	NULL		bind	NULL		interchain disulfide bond		ERp57	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_47_44838_s_226	12239218	3 Recently it has been shown that tapasin binds to ERp57 via an interchain disulfide bond, and cooperates with ERp57 in forming the correct disulfide bonds in the class I heavy chain ( 49).	bind
23591	2	7651	6	NULL	NULL	0	NULL	tapasin	NULL		cooperates with	NULL				ERp57	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_47_44838_s_226	12239218	3 Recently it has been shown that tapasin binds to ERp57 via an interchain disulfide bond, and cooperates with ERp57 in forming the correct disulfide bonds in the class I heavy chain ( 49).	bind
23592	3	7651	6	NULL	NULL	0	NULL	statement 2	NULL		forms	NULL				class I heavy chain	NULL	correct	disulfide bonds		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_47_44838_s_226	12239218	3 Recently it has been shown that tapasin binds to ERp57 via an interchain disulfide bond, and cooperates with ERp57 in forming the correct disulfide bonds in the class I heavy chain ( 49).	bind
30739	2	7652	5	13	NULL	NULL	NULL	testosterone	GP		does not result in					spin shift	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_14_9127_s_329	16467307	3 Recently, Roberts  et al. ( ) used EPR binding studies with high concentrations of P450 3A4 to suggest that the first bound molecule of testosterone does not result in a spin shift and, hence, cannot be detected by absorbance.	bind
23593	1	7652	6	NULL	NULL	0	NULL	testosterone molecule	NULL		does not result in	NULL				spin shift	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_14_9127_s_329	16467307	3 Recently, Roberts  et al. ( ) used EPR binding studies with high concentrations of P450 3A4 to suggest that the first bound molecule of testosterone does not result in a spin shift and, hence, cannot be detected by absorbance.	bind
30740	1	7653	5	13	NULL	NULL	NULL	RLI1	GP		bind					eIF2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_11_7452_s_28	16421098	3 RLI1 binds to the eukaryotic initiation factors eIF2 and eIF5 and forms part of the pre-initiation complex required for the translation of mRNA in yeast.	bind
30741	2	7653	5	13	NULL	NULL	NULL	RLI1	GP		bind					eIF5	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_11_7452_s_28	16421098	3 RLI1 binds to the eukaryotic initiation factors eIF2 and eIF5 and forms part of the pre-initiation complex required for the translation of mRNA in yeast.	bind
30742	3	7653	5	13	NULL	NULL	NULL	eIF2	GP		is a type of					eukaryotic initiation factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_11_7452_s_28	16421098	3 RLI1 binds to the eukaryotic initiation factors eIF2 and eIF5 and forms part of the pre-initiation complex required for the translation of mRNA in yeast.	bind
30743	4	7653	5	13	NULL	NULL	NULL	eIF5	GP		is a type of					eukaryotic initiation factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_11_7452_s_28	16421098	3 RLI1 binds to the eukaryotic initiation factors eIF2 and eIF5 and forms part of the pre-initiation complex required for the translation of mRNA in yeast.	bind
30744	5	7653	5	13	NULL	NULL	NULL	statement 1	Process		forms					pre-initiation complex 	GP	part of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_11_7452_s_28	16421098	3 RLI1 binds to the eukaryotic initiation factors eIF2 and eIF5 and forms part of the pre-initiation complex required for the translation of mRNA in yeast.	bind
30745	6	7653	5	13	NULL	NULL	NULL	statement 2	Process		forms					pre-initiation complex 	GP	part of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_11_7452_s_28	16421098	3 RLI1 binds to the eukaryotic initiation factors eIF2 and eIF5 and forms part of the pre-initiation complex required for the translation of mRNA in yeast.	bind
30746	7	7653	5	13	NULL	NULL	NULL	pre-initiation complex	GP		required for					mRNA	NucleicAcid	translation of			NULL	in yeast	NULL	NULL	NULL	NULL	gw70_jbiolchem_281_11_7452_s_28	16421098	3 RLI1 binds to the eukaryotic initiation factors eIF2 and eIF5 and forms part of the pre-initiation complex required for the translation of mRNA in yeast.	bind
23594	1	7653	6	NULL	NULL	0	NULL	RLI 1	NULL		bind	NULL				eIF2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_11_7452_s_28	16421098	3 RLI1 binds to the eukaryotic initiation factors eIF2 and eIF5 and forms part of the pre-initiation complex required for the translation of mRNA in yeast.	bind
23595	2	7653	6	NULL	NULL	0	NULL	RLI 1	NULL		bind	NULL				eIF5	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_11_7452_s_28	16421098	3 RLI1 binds to the eukaryotic initiation factors eIF2 and eIF5 and forms part of the pre-initiation complex required for the translation of mRNA in yeast.	bind
23596	3	7653	6	10	NULL	0	NULL	eIF2	NULL		is a type of	NULL				eukaryotic initiation factor	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_11_7452_s_28	16421098	3 RLI1 binds to the eukaryotic initiation factors eIF2 and eIF5 and forms part of the pre-initiation complex required for the translation of mRNA in yeast.	bind
23597	4	7653	6	10	NULL	0	NULL	eIF5	NULL		is a type of	NULL				eukaryotic initiation factor	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_11_7452_s_28	16421098	3 RLI1 binds to the eukaryotic initiation factors eIF2 and eIF5 and forms part of the pre-initiation complex required for the translation of mRNA in yeast.	bind
23598	5	7653	6	NULL	NULL	0	NULL	pre-initiation complex	NULL		is required for	NULL				mRNA	NULL	translation of			NULL	yeast	0	NULL	NULL	NULL	gw70_jbiolchem_281_11_7452_s_28	16421098	3 RLI1 binds to the eukaryotic initiation factors eIF2 and eIF5 and forms part of the pre-initiation complex required for the translation of mRNA in yeast.	bind
46637	6	7653	6	10	NULL	0	NULL	statement 1	NULL		forms	NULL				pre-initiation complex 	NULL	part of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_11_7452_s_28	16421098	3 RLI1 binds to the eukaryotic initiation factors eIF2 and eIF5 and forms part of the pre-initiation complex required for the translation of mRNA in yeast.	bind
46638	7	7653	6	10	NULL	0	NULL	statement 2	NULL		forms	NULL				pre-initiation complex 	NULL	part of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_11_7452_s_28	16421098	3 RLI1 binds to the eukaryotic initiation factors eIF2 and eIF5 and forms part of the pre-initiation complex required for the translation of mRNA in yeast.	bind
30747	1	7654	5	13	NULL	NULL	NULL	RyR1	GP		bind					FKBP12	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34813_s_230	9857007	3 RyR1 and RyR3 can bind both FKBP12 and FKBP12.6.	bind
30748	2	7654	5	13	NULL	NULL	NULL	RyR1	GP		bind					FKBP12.6	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34813_s_230	9857007	3 RyR1 and RyR3 can bind both FKBP12 and FKBP12.6.	bind
30749	3	7654	5	13	NULL	NULL	NULL	RyR3	GP		bind					FKBP12	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34813_s_230	9857007	3 RyR1 and RyR3 can bind both FKBP12 and FKBP12.6.	bind
30750	4	7654	5	13	NULL	NULL	NULL	RyR3	GP		bind					FKBP12.6	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34813_s_230	9857007	3 RyR1 and RyR3 can bind both FKBP12 and FKBP12.6.	bind
23599	1	7654	6	13	NULL	NULL	NULL	RyR1	GP		bind					FKBP12	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34813_s_230	9857007	3 RyR1 and RyR3 can bind both FKBP12 and FKBP12.6.	bind
23600	2	7654	6	NULL	NULL	0	NULL	RyR1	NULL		bind	NULL				FKBP12.6	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_52_34813_s_230	9857007	3 RyR1 and RyR3 can bind both FKBP12 and FKBP12.6.	bind
23601	3	7654	6	NULL	NULL	0	NULL	RyR3	NULL		bind	NULL				FKBP12	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_52_34813_s_230	9857007	3 RyR1 and RyR3 can bind both FKBP12 and FKBP12.6.	bind
23602	4	7654	6	NULL	NULL	0	NULL	RyR3	NULL		bind	NULL				FKBP12.6	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_52_34813_s_230	9857007	3 RyR1 and RyR3 can bind both FKBP12 and FKBP12.6.	bind
30751	1	7655	5	13	NULL	NULL	NULL	SNQ2	GP		encodes for					multidrug ATP-binding cassette transporter	GP	yeast plasma membrane			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_2_1511_s_147	10625705	3 SNQ2 encodes for a multidrug ATP-binding cassette transporter of the yeast plasma membrane ( 44,  45).	bind
23603	1	7655	6	10	NULL	0	NULL	SNQ2			encodes for					multidrug ATP-binding cassette transporter		yeast plasma membrane			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_2_1511_s_147	10625705	3 SNQ2 encodes for a multidrug ATP-binding cassette transporter of the yeast plasma membrane ( 44,  45).	bind
30752	1	7656	5	NULL	NULL	0	NULL		NULL		narrows	NULL		bulky helix alphaC in the alpha2I domain			NULL		collagen binding groove		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_5_3348_s_272	10652324	3 Still, it could be speculated that the bulky helix alphaC in the alpha2I domain narrows the collagen binding groove and may actually disturb the binding of type IV collagen, which contains interrupted sequences between triple helices and is therefore less compact than type I collagen.	bind
30753	2	7656	5	13	NULL	NULL	NULL	statement 1	Process		disturbs					type IV collagen	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3348_s_272	10652324	3 Still, it could be speculated that the bulky helix alphaC in the alpha2I domain narrows the collagen binding groove and may actually disturb the binding of type IV collagen, which contains interrupted sequences between triple helices and is therefore less compact than type I collagen.	bind
30754	3	7656	5	13	NULL	NULL	NULL	type IV collagen	GP		contains								interrupted sequences between triple helices		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3348_s_272	10652324	3 Still, it could be speculated that the bulky helix alphaC in the alpha2I domain narrows the collagen binding groove and may actually disturb the binding of type IV collagen, which contains interrupted sequences between triple helices and is therefore less compact than type I collagen.	bind
30755	4	7656	5	13	NULL	NULL	NULL	type IV collagen	GP		less compact than					type I collagen	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3348_s_272	10652324	3 Still, it could be speculated that the bulky helix alphaC in the alpha2I domain narrows the collagen binding groove and may actually disturb the binding of type IV collagen, which contains interrupted sequences between triple helices and is therefore less compact than type I collagen.	bind
55534	5	7656	5	13	NULL	NULL	NULL	statement 4	Process		is due to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3348_s_272	10652324	3 Still, it could be speculated that the bulky helix alphaC in the alpha2I domain narrows the collagen binding groove and may actually disturb the binding of type IV collagen, which contains interrupted sequences between triple helices and is therefore less compact than type I collagen.	bind
23622	1	7656	6	NULL	NULL	0	NULL		NULL		disturb	NULL	may	helix alphaC in the alpha2I domain		type IV collagen	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_5_3348_s_272	10652324	3 Still, it could be speculated that the bulky helix alphaC in the alpha2I domain narrows the collagen binding groove and may actually disturb the binding of type IV collagen, which contains interrupted sequences between triple helices and is therefore less compact than type I collagen.	bind
23635	2	7656	6	NULL	NULL	0	NULL	type IV collagen	NULL		contains	NULL					NULL		interrupted sequences between triple helices 		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_5_3348_s_272	10652324	3 Still, it could be speculated that the bulky helix alphaC in the alpha2I domain narrows the collagen binding groove and may actually disturb the binding of type IV collagen, which contains interrupted sequences between triple helices and is therefore less compact than type I collagen.	bind
23636	3	7656	6	NULL	NULL	0	NULL	type IV collagen	NULL		is less compact than	NULL				type I collagen	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_5_3348_s_272	10652324	3 Still, it could be speculated that the bulky helix alphaC in the alpha2I domain narrows the collagen binding groove and may actually disturb the binding of type IV collagen, which contains interrupted sequences between triple helices and is therefore less compact than type I collagen.	bind
23637	4	7656	6	NULL	NULL	0	NULL	statement 3	NULL		is due to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_5_3348_s_272	10652324	3 Still, it could be speculated that the bulky helix alphaC in the alpha2I domain narrows the collagen binding groove and may actually disturb the binding of type IV collagen, which contains interrupted sequences between triple helices and is therefore less compact than type I collagen.	bind
23642	5	7656	6	NULL	NULL	0	NULL		NULL		narrows the	NULL		helix alphaC in the alpha2I domain			NULL		collagen binding groove		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_5_3348_s_272	10652324	3 Still, it could be speculated that the bulky helix alphaC in the alpha2I domain narrows the collagen binding groove and may actually disturb the binding of type IV collagen, which contains interrupted sequences between triple helices and is therefore less compact than type I collagen.	bind
30756	1	7657	5	13	NULL	NULL	NULL	Galphai1	GP		associates with					RGS4	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_3_1269_s_111	9430654	3 Superposition of the structure of Galphai1 associated with RGS4 on that of Galphas associated with adenylyl cyclase suggests that the interaction of an RGS protein with a G protein alpha subunit would not block binding of a Galpha protein to adenylyl cyclase.	bind
30757	2	7657	5	13	NULL	NULL	NULL	Galphas	GP		associates with					adenylyl cyclase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_3_1269_s_111	9430654	3 Superposition of the structure of Galphai1 associated with RGS4 on that of Galphas associated with adenylyl cyclase suggests that the interaction of an RGS protein with a G protein alpha subunit would not block binding of a Galpha protein to adenylyl cyclase.	bind
30758	3	7657	5	13	NULL	NULL	NULL	RGS protein	GP		interacts with					G protein	GP		alpha subunit		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_3_1269_s_111	9430654	3 Superposition of the structure of Galphai1 associated with RGS4 on that of Galphas associated with adenylyl cyclase suggests that the interaction of an RGS protein with a G protein alpha subunit would not block binding of a Galpha protein to adenylyl cyclase.	bind
30759	4	7657	5	13	NULL	NULL	NULL	Galpha protein	GP		bind					adenylyl cyclase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_3_1269_s_111	9430654	3 Superposition of the structure of Galphai1 associated with RGS4 on that of Galphas associated with adenylyl cyclase suggests that the interaction of an RGS protein with a G protein alpha subunit would not block binding of a Galpha protein to adenylyl cyclase.	bind
30760	5	7657	5	13	NULL	NULL	NULL	statement 3	Process		does not block					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_3_1269_s_111	9430654	3 Superposition of the structure of Galphai1 associated with RGS4 on that of Galphas associated with adenylyl cyclase suggests that the interaction of an RGS protein with a G protein alpha subunit would not block binding of a Galpha protein to adenylyl cyclase.	bind
23790	1	7657	6	10	NULL	0	NULL	RGS protein	NULL		interacts with	NULL				G protein 	NULL		alpha subunit		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_3_1269_s_111	9430654	3 Superposition of the structure of Galphai1 associated with RGS4 on that of Galphas associated with adenylyl cyclase suggests that the interaction of an RGS protein with a G protein alpha subunit would not block binding of a Galpha protein to adenylyl cyclase.	bind
23791	2	7657	6	NULL	NULL	0	NULL	Galpha protein	NULL		bind	NULL				adenylyl cyclase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_3_1269_s_111	9430654	3 Superposition of the structure of Galphai1 associated with RGS4 on that of Galphas associated with adenylyl cyclase suggests that the interaction of an RGS protein with a G protein alpha subunit would not block binding of a Galpha protein to adenylyl cyclase.	bind
23792	3	7657	6	10	NULL	0	NULL	statement 1	NULL		does not block	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_3_1269_s_111	9430654	3 Superposition of the structure of Galphai1 associated with RGS4 on that of Galphas associated with adenylyl cyclase suggests that the interaction of an RGS protein with a G protein alpha subunit would not block binding of a Galpha protein to adenylyl cyclase.	bind
24573	4	7657	6	NULL	NULL	0	NULL	Galphai1	NULL		associates with	NULL				RGS4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_3_1269_s_111	9430654	3 Superposition of the structure of Galphai1 associated with RGS4 on that of Galphas associated with adenylyl cyclase suggests that the interaction of an RGS protein with a G protein alpha subunit would not block binding of a Galpha protein to adenylyl cyclase.	bind
46639	5	7657	6	10	NULL	0	NULL	Galphas	NULL		associate with	NULL				adenylyl cyclase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_3_1269_s_111	9430654	3 Superposition of the structure of Galphai1 associated with RGS4 on that of Galphas associated with adenylyl cyclase suggests that the interaction of an RGS protein with a G protein alpha subunit would not block binding of a Galpha protein to adenylyl cyclase.	bind
30761	1	7659	5	13	NULL	NULL	NULL	Eps8	GP		bind					Etk	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_52_41124_s_283	11013262	3 The binding of Eps8 to Etk also increases the kinase activity of Etk.	bind
30762	2	7659	5	13	NULL	NULL	NULL	statement 1	Process		increase					Etk	GP	kinase activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_52_41124_s_283	11013262	3 The binding of Eps8 to Etk also increases the kinase activity of Etk.	bind
23643	1	7659	6	NULL	NULL	0	NULL	Eps8	NULL		bind	NULL				Etk	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_52_41124_s_283	11013262	3 The binding of Eps8 to Etk also increases the kinase activity of Etk.	bind
23645	2	7659	6	NULL	NULL	0	NULL	statement 1	NULL		increases	NULL				Etk	NULL	kinase activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_52_41124_s_283	11013262	3 The binding of Eps8 to Etk also increases the kinase activity of Etk.	bind
30763	1	7660	5	13	NULL	NULL	NULL	TrfA protein	GP		bind					RK2	GP			iterons at minimal origin of replication	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_20173_s_71	9242693	3 The binding of the TrfA protein to the iterons at the minimal RK2 origin of replication has been characterized in detail ( 25,  26,  37,  40); however, little is known about the nature of binding of the DnaA protein to  oriV.	bind
46640	2	7660	5	13	NULL	NULL	NULL	DnaA protein	GP		bind					oriV	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_20173_s_71	9242693	3 The binding of the TrfA protein to the iterons at the minimal RK2 origin of replication has been characterized in detail ( 25,  26,  37,  40); however, little is known about the nature of binding of the DnaA protein to  oriV.	bind
23647	1	7660	6	10	NULL	0	NULL	TrfA protein	NULL		bind	NULL				RK2	NULL			iterons at minimal  origin of replication	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_20173_s_71	9242693	3 The binding of the TrfA protein to the iterons at the minimal RK2 origin of replication has been characterized in detail ( 25,  26,  37,  40); however, little is known about the nature of binding of the DnaA protein to  oriV.	bind
23648	2	7660	6	NULL	NULL	0	NULL	DnaA protein	NULL		bind	NULL				oriV	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_32_20173_s_71	9242693	3 The binding of the TrfA protein to the iterons at the minimal RK2 origin of replication has been characterized in detail ( 25,  26,  37,  40); however, little is known about the nature of binding of the DnaA protein to  oriV.	bind
30764	1	7662	5	13	NULL	NULL	NULL	pemphigus antibody	GP		targets					alpha9	GP	keratinocyte			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_4_1377_s_262	11021840	3 The fact that keratinocyte alpha9 is targeted by pemphigus antibody is also in keeping with the notion that the biochemical events elicited because of PV IgG binding to the keratinocyte cell surface include both the nicotinic-like effects (ie, Ca2+ influx) and the muscarinic-like effects (ie, activation of phospholipase C, production of inositol 1,4,5-trisphosphate, rapid transient increase of intracellular Ca2+, changes in the intracellular cAMP/cGMP ratios, and activation and translocation of protein kinase C from the cytosol to the particulate/cytoskeletal fractions).	bind
30765	2	7662	5	13	NULL	NULL	NULL	PV IgG	GP		bind					cell surface	CellComponent	keratinocyte			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_4_1377_s_262	11021840	3 The fact that keratinocyte alpha9 is targeted by pemphigus antibody is also in keeping with the notion that the biochemical events elicited because of PV IgG binding to the keratinocyte cell surface include both the nicotinic-like effects (ie, Ca2+ influx) and the muscarinic-like effects (ie, activation of phospholipase C, production of inositol 1,4,5-trisphosphate, rapid transient increase of intracellular Ca2+, changes in the intracellular cAMP/cGMP ratios, and activation and translocation of protein kinase C from the cytosol to the particulate/cytoskeletal fractions).	bind
30766	3	7662	5	13	NULL	NULL	NULL	statement 2	Process		elicits					Ca2+ influx	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_4_1377_s_262	11021840	3 The fact that keratinocyte alpha9 is targeted by pemphigus antibody is also in keeping with the notion that the biochemical events elicited because of PV IgG binding to the keratinocyte cell surface include both the nicotinic-like effects (ie, Ca2+ influx) and the muscarinic-like effects (ie, activation of phospholipase C, production of inositol 1,4,5-trisphosphate, rapid transient increase of intracellular Ca2+, changes in the intracellular cAMP/cGMP ratios, and activation and translocation of protein kinase C from the cytosol to the particulate/cytoskeletal fractions).	bind
30767	4	7662	5	13	NULL	NULL	NULL	Ca2+ influx	Process		is a type of					nicotinic-like effects	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_4_1377_s_262	11021840	3 The fact that keratinocyte alpha9 is targeted by pemphigus antibody is also in keeping with the notion that the biochemical events elicited because of PV IgG binding to the keratinocyte cell surface include both the nicotinic-like effects (ie, Ca2+ influx) and the muscarinic-like effects (ie, activation of phospholipase C, production of inositol 1,4,5-trisphosphate, rapid transient increase of intracellular Ca2+, changes in the intracellular cAMP/cGMP ratios, and activation and translocation of protein kinase C from the cytosol to the particulate/cytoskeletal fractions).	bind
30768	5	7662	5	13	NULL	NULL	NULL	statement 2	Process		elicits					phospholipase C	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_4_1377_s_262	11021840	3 The fact that keratinocyte alpha9 is targeted by pemphigus antibody is also in keeping with the notion that the biochemical events elicited because of PV IgG binding to the keratinocyte cell surface include both the nicotinic-like effects (ie, Ca2+ influx) and the muscarinic-like effects (ie, activation of phospholipase C, production of inositol 1,4,5-trisphosphate, rapid transient increase of intracellular Ca2+, changes in the intracellular cAMP/cGMP ratios, and activation and translocation of protein kinase C from the cytosol to the particulate/cytoskeletal fractions).	bind
30769	6	7662	5	13	NULL	NULL	NULL	statement 2	Process		elicits					inositol 1,4,5-trisphosphate	Chemical	production of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_4_1377_s_262	11021840	3 The fact that keratinocyte alpha9 is targeted by pemphigus antibody is also in keeping with the notion that the biochemical events elicited because of PV IgG binding to the keratinocyte cell surface include both the nicotinic-like effects (ie, Ca2+ influx) and the muscarinic-like effects (ie, activation of phospholipase C, production of inositol 1,4,5-trisphosphate, rapid transient increase of intracellular Ca2+, changes in the intracellular cAMP/cGMP ratios, and activation and translocation of protein kinase C from the cytosol to the particulate/cytoskeletal fractions).	bind
30770	7	7662	5	13	NULL	NULL	NULL	statement 2	Process		elicits					Ca2+	Chemical	rapid transient increase of intracellular			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_4_1377_s_262	11021840	3 The fact that keratinocyte alpha9 is targeted by pemphigus antibody is also in keeping with the notion that the biochemical events elicited because of PV IgG binding to the keratinocyte cell surface include both the nicotinic-like effects (ie, Ca2+ influx) and the muscarinic-like effects (ie, activation of phospholipase C, production of inositol 1,4,5-trisphosphate, rapid transient increase of intracellular Ca2+, changes in the intracellular cAMP/cGMP ratios, and activation and translocation of protein kinase C from the cytosol to the particulate/cytoskeletal fractions).	bind
30771	8	7662	5	13	NULL	NULL	NULL	statement 2	Process		elicits					cAMP/cGMP ratios	Chemical	changes in intracellular			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_4_1377_s_262	11021840	3 The fact that keratinocyte alpha9 is targeted by pemphigus antibody is also in keeping with the notion that the biochemical events elicited because of PV IgG binding to the keratinocyte cell surface include both the nicotinic-like effects (ie, Ca2+ influx) and the muscarinic-like effects (ie, activation of phospholipase C, production of inositol 1,4,5-trisphosphate, rapid transient increase of intracellular Ca2+, changes in the intracellular cAMP/cGMP ratios, and activation and translocation of protein kinase C from the cytosol to the particulate/cytoskeletal fractions).	bind
30772	9	7662	5	13	NULL	NULL	NULL	statement 2	Process		elicits					protein kinase C	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_4_1377_s_262	11021840	3 The fact that keratinocyte alpha9 is targeted by pemphigus antibody is also in keeping with the notion that the biochemical events elicited because of PV IgG binding to the keratinocyte cell surface include both the nicotinic-like effects (ie, Ca2+ influx) and the muscarinic-like effects (ie, activation of phospholipase C, production of inositol 1,4,5-trisphosphate, rapid transient increase of intracellular Ca2+, changes in the intracellular cAMP/cGMP ratios, and activation and translocation of protein kinase C from the cytosol to the particulate/cytoskeletal fractions).	bind
30773	10	7662	5	13	NULL	NULL	NULL	protein kinase C	GP	activated	 translocates from					cytosol	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_4_1377_s_262	11021840	3 The fact that keratinocyte alpha9 is targeted by pemphigus antibody is also in keeping with the notion that the biochemical events elicited because of PV IgG binding to the keratinocyte cell surface include both the nicotinic-like effects (ie, Ca2+ influx) and the muscarinic-like effects (ie, activation of phospholipase C, production of inositol 1,4,5-trisphosphate, rapid transient increase of intracellular Ca2+, changes in the intracellular cAMP/cGMP ratios, and activation and translocation of protein kinase C from the cytosol to the particulate/cytoskeletal fractions).	bind
30774	12	7662	5	13	NULL	NULL	NULL	phospholipase C	GP	activation of	is a type of					muscarinic-like effects	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_4_1377_s_262	11021840	3 The fact that keratinocyte alpha9 is targeted by pemphigus antibody is also in keeping with the notion that the biochemical events elicited because of PV IgG binding to the keratinocyte cell surface include both the nicotinic-like effects (ie, Ca2+ influx) and the muscarinic-like effects (ie, activation of phospholipase C, production of inositol 1,4,5-trisphosphate, rapid transient increase of intracellular Ca2+, changes in the intracellular cAMP/cGMP ratios, and activation and translocation of protein kinase C from the cytosol to the particulate/cytoskeletal fractions).	bind
30775	13	7662	5	13	NULL	NULL	NULL	inositol 1,4,5-trisphosphate	Chemical	production of	is a type of					muscarinic-like effects	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_4_1377_s_262	11021840	3 The fact that keratinocyte alpha9 is targeted by pemphigus antibody is also in keeping with the notion that the biochemical events elicited because of PV IgG binding to the keratinocyte cell surface include both the nicotinic-like effects (ie, Ca2+ influx) and the muscarinic-like effects (ie, activation of phospholipase C, production of inositol 1,4,5-trisphosphate, rapid transient increase of intracellular Ca2+, changes in the intracellular cAMP/cGMP ratios, and activation and translocation of protein kinase C from the cytosol to the particulate/cytoskeletal fractions).	bind
30776	14	7662	5	13	NULL	NULL	NULL	Ca2+	Chemical	rapid transient increase of intracellular	is a type of					muscarinic-like effects	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_4_1377_s_262	11021840	3 The fact that keratinocyte alpha9 is targeted by pemphigus antibody is also in keeping with the notion that the biochemical events elicited because of PV IgG binding to the keratinocyte cell surface include both the nicotinic-like effects (ie, Ca2+ influx) and the muscarinic-like effects (ie, activation of phospholipase C, production of inositol 1,4,5-trisphosphate, rapid transient increase of intracellular Ca2+, changes in the intracellular cAMP/cGMP ratios, and activation and translocation of protein kinase C from the cytosol to the particulate/cytoskeletal fractions).	bind
30777	15	7662	5	13	NULL	NULL	NULL	cAMP/cGMP ratios	Chemical	changes in intracellular	is a type of					muscarinic-like effects	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_4_1377_s_262	11021840	3 The fact that keratinocyte alpha9 is targeted by pemphigus antibody is also in keeping with the notion that the biochemical events elicited because of PV IgG binding to the keratinocyte cell surface include both the nicotinic-like effects (ie, Ca2+ influx) and the muscarinic-like effects (ie, activation of phospholipase C, production of inositol 1,4,5-trisphosphate, rapid transient increase of intracellular Ca2+, changes in the intracellular cAMP/cGMP ratios, and activation and translocation of protein kinase C from the cytosol to the particulate/cytoskeletal fractions).	bind
30778	16	7662	5	13	NULL	NULL	NULL	protein kinase C	GP	activation of	is a type of					muscarinic-like effects	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_4_1377_s_262	11021840	3 The fact that keratinocyte alpha9 is targeted by pemphigus antibody is also in keeping with the notion that the biochemical events elicited because of PV IgG binding to the keratinocyte cell surface include both the nicotinic-like effects (ie, Ca2+ influx) and the muscarinic-like effects (ie, activation of phospholipase C, production of inositol 1,4,5-trisphosphate, rapid transient increase of intracellular Ca2+, changes in the intracellular cAMP/cGMP ratios, and activation and translocation of protein kinase C from the cytosol to the particulate/cytoskeletal fractions).	bind
30779	17	7662	5	13	NULL	NULL	NULL	protein kinase C	GP	translocation of	is a type of					muscarinic-like effects	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_4_1377_s_262	11021840	3 The fact that keratinocyte alpha9 is targeted by pemphigus antibody is also in keeping with the notion that the biochemical events elicited because of PV IgG binding to the keratinocyte cell surface include both the nicotinic-like effects (ie, Ca2+ influx) and the muscarinic-like effects (ie, activation of phospholipase C, production of inositol 1,4,5-trisphosphate, rapid transient increase of intracellular Ca2+, changes in the intracellular cAMP/cGMP ratios, and activation and translocation of protein kinase C from the cytosol to the particulate/cytoskeletal fractions).	bind
46641	11	7662	5	13	NULL	NULL	NULL	protein kinase C	GP		translocates to					particulate/cytoskeletal fractions	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_4_1377_s_262	11021840	3 The fact that keratinocyte alpha9 is targeted by pemphigus antibody is also in keeping with the notion that the biochemical events elicited because of PV IgG binding to the keratinocyte cell surface include both the nicotinic-like effects (ie, Ca2+ influx) and the muscarinic-like effects (ie, activation of phospholipase C, production of inositol 1,4,5-trisphosphate, rapid transient increase of intracellular Ca2+, changes in the intracellular cAMP/cGMP ratios, and activation and translocation of protein kinase C from the cytosol to the particulate/cytoskeletal fractions).	bind
23649	1	7662	6	NULL	NULL	0	NULL	pemphigus antibody	NULL		targets	NULL				keratinocyte alpha9	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_4_1377_s_262	11021840	3 The fact that keratinocyte alpha9 is targeted by pemphigus antibody is also in keeping with the notion that the biochemical events elicited because of PV IgG binding to the keratinocyte cell surface include both the nicotinic-like effects (ie, Ca2+ influx) and the muscarinic-like effects (ie, activation of phospholipase C, production of inositol 1,4,5-trisphosphate, rapid transient increase of intracellular Ca2+, changes in the intracellular cAMP/cGMP ratios, and activation and translocation of protein kinase C from the cytosol to the particulate/cytoskeletal fractions).	bind
23650	2	7662	6	NULL	NULL	0	NULL	PV IgG	NULL		bind	NULL				keratinocyte cell surface	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_4_1377_s_262	11021840	3 The fact that keratinocyte alpha9 is targeted by pemphigus antibody is also in keeping with the notion that the biochemical events elicited because of PV IgG binding to the keratinocyte cell surface include both the nicotinic-like effects (ie, Ca2+ influx) and the muscarinic-like effects (ie, activation of phospholipase C, production of inositol 1,4,5-trisphosphate, rapid transient increase of intracellular Ca2+, changes in the intracellular cAMP/cGMP ratios, and activation and translocation of protein kinase C from the cytosol to the particulate/cytoskeletal fractions).	bind
23653	3	7662	6	NULL	NULL	0	NULL	statement 2	NULL		elicits	NULL				nicotinic-like effects	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_4_1377_s_262	11021840	3 The fact that keratinocyte alpha9 is targeted by pemphigus antibody is also in keeping with the notion that the biochemical events elicited because of PV IgG binding to the keratinocyte cell surface include both the nicotinic-like effects (ie, Ca2+ influx) and the muscarinic-like effects (ie, activation of phospholipase C, production of inositol 1,4,5-trisphosphate, rapid transient increase of intracellular Ca2+, changes in the intracellular cAMP/cGMP ratios, and activation and translocation of protein kinase C from the cytosol to the particulate/cytoskeletal fractions).	bind
23654	4	7662	6	NULL	NULL	0	NULL	statement 2	NULL		elicits	NULL				muscarinic-like effects	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_4_1377_s_262	11021840	3 The fact that keratinocyte alpha9 is targeted by pemphigus antibody is also in keeping with the notion that the biochemical events elicited because of PV IgG binding to the keratinocyte cell surface include both the nicotinic-like effects (ie, Ca2+ influx) and the muscarinic-like effects (ie, activation of phospholipase C, production of inositol 1,4,5-trisphosphate, rapid transient increase of intracellular Ca2+, changes in the intracellular cAMP/cGMP ratios, and activation and translocation of protein kinase C from the cytosol to the particulate/cytoskeletal fractions).	bind
23655	5	7662	6	10	NULL	0	NULL	Ca2+ influx	NULL		is a type of	NULL				nicotinic-like effect	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_4_1377_s_262	11021840	3 The fact that keratinocyte alpha9 is targeted by pemphigus antibody is also in keeping with the notion that the biochemical events elicited because of PV IgG binding to the keratinocyte cell surface include both the nicotinic-like effects (ie, Ca2+ influx) and the muscarinic-like effects (ie, activation of phospholipase C, production of inositol 1,4,5-trisphosphate, rapid transient increase of intracellular Ca2+, changes in the intracellular cAMP/cGMP ratios, and activation and translocation of protein kinase C from the cytosol to the particulate/cytoskeletal fractions).	bind
23656	6	7662	6	10	NULL	0	NULL	phospholipase C	NULL	activation of 	is a type of	NULL				muscarinic-like effect	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_4_1377_s_262	11021840	3 The fact that keratinocyte alpha9 is targeted by pemphigus antibody is also in keeping with the notion that the biochemical events elicited because of PV IgG binding to the keratinocyte cell surface include both the nicotinic-like effects (ie, Ca2+ influx) and the muscarinic-like effects (ie, activation of phospholipase C, production of inositol 1,4,5-trisphosphate, rapid transient increase of intracellular Ca2+, changes in the intracellular cAMP/cGMP ratios, and activation and translocation of protein kinase C from the cytosol to the particulate/cytoskeletal fractions).	bind
23657	7	7662	6	10	NULL	0	NULL	inositol 1,4,5-trisphosphate	NULL	production of	is a type of	NULL				muscarinic-like effect	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_4_1377_s_262	11021840	3 The fact that keratinocyte alpha9 is targeted by pemphigus antibody is also in keeping with the notion that the biochemical events elicited because of PV IgG binding to the keratinocyte cell surface include both the nicotinic-like effects (ie, Ca2+ influx) and the muscarinic-like effects (ie, activation of phospholipase C, production of inositol 1,4,5-trisphosphate, rapid transient increase of intracellular Ca2+, changes in the intracellular cAMP/cGMP ratios, and activation and translocation of protein kinase C from the cytosol to the particulate/cytoskeletal fractions).	bind
23659	8	7662	6	10	NULL	0	NULL	intracellular Ca2+	NULL	transient increase of	is a type of	NULL				muscarinic-like effect	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_4_1377_s_262	11021840	3 The fact that keratinocyte alpha9 is targeted by pemphigus antibody is also in keeping with the notion that the biochemical events elicited because of PV IgG binding to the keratinocyte cell surface include both the nicotinic-like effects (ie, Ca2+ influx) and the muscarinic-like effects (ie, activation of phospholipase C, production of inositol 1,4,5-trisphosphate, rapid transient increase of intracellular Ca2+, changes in the intracellular cAMP/cGMP ratios, and activation and translocation of protein kinase C from the cytosol to the particulate/cytoskeletal fractions).	bind
23660	9	7662	6	10	NULL	0	NULL	intracellular cAMP/cGMP ratio	NULL	changes in	is a type of	NULL				muscarinic-like effect	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_4_1377_s_262	11021840	3 The fact that keratinocyte alpha9 is targeted by pemphigus antibody is also in keeping with the notion that the biochemical events elicited because of PV IgG binding to the keratinocyte cell surface include both the nicotinic-like effects (ie, Ca2+ influx) and the muscarinic-like effects (ie, activation of phospholipase C, production of inositol 1,4,5-trisphosphate, rapid transient increase of intracellular Ca2+, changes in the intracellular cAMP/cGMP ratios, and activation and translocation of protein kinase C from the cytosol to the particulate/cytoskeletal fractions).	bind
23661	11	7662	6	10	NULL	0	NULL	protein kinase C	NULL		 translocates to	NULL				particulate/cytoskeletal fraction	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_4_1377_s_262	11021840	3 The fact that keratinocyte alpha9 is targeted by pemphigus antibody is also in keeping with the notion that the biochemical events elicited because of PV IgG binding to the keratinocyte cell surface include both the nicotinic-like effects (ie, Ca2+ influx) and the muscarinic-like effects (ie, activation of phospholipase C, production of inositol 1,4,5-trisphosphate, rapid transient increase of intracellular Ca2+, changes in the intracellular cAMP/cGMP ratios, and activation and translocation of protein kinase C from the cytosol to the particulate/cytoskeletal fractions).	bind
23662	12	7662	6	10	NULL	0	NULL	statement 10	NULL		is a type of	NULL				muscarinic-like effect	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_4_1377_s_262	11021840	3 The fact that keratinocyte alpha9 is targeted by pemphigus antibody is also in keeping with the notion that the biochemical events elicited because of PV IgG binding to the keratinocyte cell surface include both the nicotinic-like effects (ie, Ca2+ influx) and the muscarinic-like effects (ie, activation of phospholipase C, production of inositol 1,4,5-trisphosphate, rapid transient increase of intracellular Ca2+, changes in the intracellular cAMP/cGMP ratios, and activation and translocation of protein kinase C from the cytosol to the particulate/cytoskeletal fractions).	bind
23663	13	7662	6	10	NULL	0	NULL	protein kinase C	NULL	activation of	is a type of	NULL				muscarinic-like effect	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_4_1377_s_262	11021840	3 The fact that keratinocyte alpha9 is targeted by pemphigus antibody is also in keeping with the notion that the biochemical events elicited because of PV IgG binding to the keratinocyte cell surface include both the nicotinic-like effects (ie, Ca2+ influx) and the muscarinic-like effects (ie, activation of phospholipase C, production of inositol 1,4,5-trisphosphate, rapid transient increase of intracellular Ca2+, changes in the intracellular cAMP/cGMP ratios, and activation and translocation of protein kinase C from the cytosol to the particulate/cytoskeletal fractions).	bind
46642	10	7662	6	10	NULL	0	NULL	protein kinase C	NULL		translocates from	NULL				 cytosol	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_4_1377_s_262	11021840	3 The fact that keratinocyte alpha9 is targeted by pemphigus antibody is also in keeping with the notion that the biochemical events elicited because of PV IgG binding to the keratinocyte cell surface include both the nicotinic-like effects (ie, Ca2+ influx) and the muscarinic-like effects (ie, activation of phospholipase C, production of inositol 1,4,5-trisphosphate, rapid transient increase of intracellular Ca2+, changes in the intracellular cAMP/cGMP ratios, and activation and translocation of protein kinase C from the cytosol to the particulate/cytoskeletal fractions).	bind
30780	1	7663	5	13	NULL	NULL	NULL	p185deltaC	GP		stimulates					cell migration	Process	spontaneous			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_31_28954_s_235	11387320	3 The finding that p185deltaC is capable of stimulating spontaneous cell migration and inducing CML-like disease in BMT mice is consistent with the results reported by other investigators that the direct binding of Crkl to Bcr-Abl is not required for Bcr-Abl transformation ( 42).	bind
30781	2	7663	5	13	NULL	NULL	NULL	p185deltaC	GP		induces					CML-like disease	MedicalFinding				NULL	in BMT mice	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_31_28954_s_235	11387320	3 The finding that p185deltaC is capable of stimulating spontaneous cell migration and inducing CML-like disease in BMT mice is consistent with the results reported by other investigators that the direct binding of Crkl to Bcr-Abl is not required for Bcr-Abl transformation ( 42).	bind
30782	3	7663	5	13	NULL	NULL	NULL	Crkl	GP		bind		directly			Bcr-Abl	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_31_28954_s_235	11387320	3 The finding that p185deltaC is capable of stimulating spontaneous cell migration and inducing CML-like disease in BMT mice is consistent with the results reported by other investigators that the direct binding of Crkl to Bcr-Abl is not required for Bcr-Abl transformation ( 42).	bind
30783	4	7663	5	13	NULL	NULL	NULL	statement 3	Process		is not required for					Bcr-Abl	GP	 transformation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_31_28954_s_235	11387320	3 The finding that p185deltaC is capable of stimulating spontaneous cell migration and inducing CML-like disease in BMT mice is consistent with the results reported by other investigators that the direct binding of Crkl to Bcr-Abl is not required for Bcr-Abl transformation ( 42).	bind
23664	1	7663	6	NULL	NULL	0	NULL	p185deltaC	NULL		stimulates	NULL				cell migration	NULL	spontaneous			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_31_28954_s_235	11387320	3 The finding that p185deltaC is capable of stimulating spontaneous cell migration and inducing CML-like disease in BMT mice is consistent with the results reported by other investigators that the direct binding of Crkl to Bcr-Abl is not required for Bcr-Abl transformation ( 42).	bind
23666	2	7663	6	NULL	NULL	0	NULL	p185deltaC	NULL		induce	NULL				CML-like disease	NULL				NULL	BMT mice	0	NULL	NULL	NULL	gw60_jbiolchem_276_31_28954_s_235	11387320	3 The finding that p185deltaC is capable of stimulating spontaneous cell migration and inducing CML-like disease in BMT mice is consistent with the results reported by other investigators that the direct binding of Crkl to Bcr-Abl is not required for Bcr-Abl transformation ( 42).	bind
23667	3	7663	6	NULL	NULL	0	NULL	Crkl	NULL		bind	NULL	directly			Bcr-Abl	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_31_28954_s_235	11387320	3 The finding that p185deltaC is capable of stimulating spontaneous cell migration and inducing CML-like disease in BMT mice is consistent with the results reported by other investigators that the direct binding of Crkl to Bcr-Abl is not required for Bcr-Abl transformation ( 42).	bind
23668	4	7663	6	NULL	NULL	0	NULL	statement 3	NULL		is not required for	NULL				Bcr-Abl	NULL	transformation of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_31_28954_s_235	11387320	3 The finding that p185deltaC is capable of stimulating spontaneous cell migration and inducing CML-like disease in BMT mice is consistent with the results reported by other investigators that the direct binding of Crkl to Bcr-Abl is not required for Bcr-Abl transformation ( 42).	bind
30784	1	7664	5	13	NULL	NULL	NULL	galectins	GP		bind		specifically			beta-galactoside derivatives	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_5_1601_s_15	10329612	3 The first class comprises a family of small molecular mass proteins named galectins that specifically bind to beta-galactoside derivatives in a calcium-independent manner.	bind
30785	2	7664	5	13	NULL	NULL	NULL	statement 1	Process		is independent of					calcium	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_5_1601_s_15	10329612	3 The first class comprises a family of small molecular mass proteins named galectins that specifically bind to beta-galactoside derivatives in a calcium-independent manner.	bind
30786	3	7664	5	13	NULL	NULL	NULL	galectins	GP		is a type of					small molecular mass proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_5_1601_s_15	10329612	3 The first class comprises a family of small molecular mass proteins named galectins that specifically bind to beta-galactoside derivatives in a calcium-independent manner.	bind
23672	1	7664	6	NULL	NULL	0	NULL	galectins	NULL		bind	NULL	specifically			beta-galactoside derivatives	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_5_1601_s_15	10329612	3 The first class comprises a family of small molecular mass proteins named galectins that specifically bind to beta-galactoside derivatives in a calcium-independent manner.	bind
23673	2	7664	6	10	NULL	0	NULL	galectins	NULL		is a type of	NULL				small molecular mass proteins	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_5_1601_s_15	10329612	3 The first class comprises a family of small molecular mass proteins named galectins that specifically bind to beta-galactoside derivatives in a calcium-independent manner.	bind
23674	3	7664	6	NULL	NULL	0	NULL	statement 1	NULL		is independent of	NULL				calcium	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_5_1601_s_15	10329612	3 The first class comprises a family of small molecular mass proteins named galectins that specifically bind to beta-galactoside derivatives in a calcium-independent manner.	bind
30787	1	7665	5	13	NULL	NULL	NULL	Fra-2	GP		is a type of					Fos-related antigen	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_24_17991_s_281	10747965	3 The Fos-related antigen, Fra-2, that can bind to the PF1 site ( 19) was also tested for its ability to regulate  p53 promoter activity.	bind
30788	2	7665	5	13	NULL	NULL	NULL	Fra-2	GP		bind									PF1 site	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_24_17991_s_281	10747965	3 The Fos-related antigen, Fra-2, that can bind to the PF1 site ( 19) was also tested for its ability to regulate  p53 promoter activity.	bind
23677	1	7665	6	NULL	NULL	0	NULL	Fra-2	NULL		bind	NULL					NULL			PF1 site	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_24_17991_s_281	10747965	3 The Fos-related antigen, Fra-2, that can bind to the PF1 site ( 19) was also tested for its ability to regulate  p53 promoter activity.	bind
23680	2	7665	6	10	NULL	0	NULL	Fra-2	NULL		is a type of	NULL				Fos-related antigen	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_24_17991_s_281	10747965	3 The Fos-related antigen, Fra-2, that can bind to the PF1 site ( 19) was also tested for its ability to regulate  p53 promoter activity.	bind
30789	1	7668	5	13	NULL	NULL	NULL	NF-kappaB	GP		bind					TAFII105alpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_48_44963_s_185	11567023	3 The proximity of these domains raised the possibility that NF-kappaB binding and nuclear export protein binding with TAFII105alpha may be mutually exclusive.	bind
30790	2	7668	5	13	NULL	NULL	NULL	nuclear export protein	GP		bind					TAFII105alpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_48_44963_s_185	11567023	3 The proximity of these domains raised the possibility that NF-kappaB binding and nuclear export protein binding with TAFII105alpha may be mutually exclusive.	bind
30791	3	7668	5	13	NULL	NULL	NULL	statement 1	Process		is mutually exclusive to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_48_44963_s_185	11567023	3 The proximity of these domains raised the possibility that NF-kappaB binding and nuclear export protein binding with TAFII105alpha may be mutually exclusive.	bind
23794	1	7668	6	NULL	NULL	0	NULL	NF-kappaB	NULL		bind	NULL				TAFII105alpha	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_48_44963_s_185	11567023	3 The proximity of these domains raised the possibility that NF-kappaB binding and nuclear export protein binding with TAFII105alpha may be mutually exclusive.	bind
23795	2	7668	6	NULL	NULL	0	NULL	nuclear export protein	NULL		bind	NULL				TAFII105alpha	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_48_44963_s_185	11567023	3 The proximity of these domains raised the possibility that NF-kappaB binding and nuclear export protein binding with TAFII105alpha may be mutually exclusive.	bind
23796	3	7668	6	NULL	NULL	0	NULL	statement 1	NULL		is independent of	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_48_44963_s_185	11567023	3 The proximity of these domains raised the possibility that NF-kappaB binding and nuclear export protein binding with TAFII105alpha may be mutually exclusive.	bind
30792	1	7669	5	13	NULL	NULL	NULL	ATP	Chemical		does not stabilize					TAP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14632_s_196	10329656	3 The reason for the lack of TAP stabilization by ATP reported by Russ ( 21) is less evident; it is possible that Triton or Nonidet P-40-solubilized TAP proteins bind ATP with reduced affinity allowing for labeling with photoreactive ATP analogues, but not stabilization of TAP structure.	bind
30793	2	7669	5	13	NULL	NULL	NULL	TAP proteins	GP	solubilized	bind		low affinity			ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14632_s_196	10329656	3 The reason for the lack of TAP stabilization by ATP reported by Russ ( 21) is less evident; it is possible that Triton or Nonidet P-40-solubilized TAP proteins bind ATP with reduced affinity allowing for labeling with photoreactive ATP analogues, but not stabilization of TAP structure.	bind
23797	1	7669	6	10	NULL	0	NULL	TAP protein	NULL	solubilized	bind	NULL	low affinity			ATP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14632_s_196	10329656	3 The reason for the lack of TAP stabilization by ATP reported by Russ ( 21) is less evident; it is possible that Triton or Nonidet P-40-solubilized TAP proteins bind ATP with reduced affinity allowing for labeling with photoreactive ATP analogues, but not stabilization of TAP structure.	bind
23798	2	7669	6	NULL	NULL	0	NULL	statement 1	NULL		does not stabilize	NULL				TAP	NULL	structure of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_21_14632_s_196	10329656	3 The reason for the lack of TAP stabilization by ATP reported by Russ ( 21) is less evident; it is possible that Triton or Nonidet P-40-solubilized TAP proteins bind ATP with reduced affinity allowing for labeling with photoreactive ATP analogues, but not stabilization of TAP structure.	bind
30794	1	7670	5	13	NULL	NULL	NULL	PDK	GP		bind								GST-lipoyl domains		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15773_s_383	10748134	3 The use of commercially available thrombin preparations to remove His tags from the PDKs caused problems in subsequent studies analyzing PDK binding to GST-lipoyl domains  .	bind
23799	1	7670	6	NULL	NULL	0	NULL	PDK	NULL		bind	NULL					NULL		GST-lipoyl domains		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15773_s_383	10748134	3 The use of commercially available thrombin preparations to remove His tags from the PDKs caused problems in subsequent studies analyzing PDK binding to GST-lipoyl domains  .	bind
30795	1	7671	5	13	NULL	NULL	NULL	EIIIA segment	GP		bind					alpha4beta1	GP				NULL	in MOLT-3 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_14467_s_260	11839764	3 Therefore it is of interest that we observe (Fig.  6) that the interaction of EIIIA segment with alpha4beta1 in MOLT-3 cells increases phosphorylation of p44/42 MAP kinase.	bind
30796	2	7671	5	13	NULL	NULL	NULL	statement 1	Process		increases					p44/42 MAP kinase	GP	phosphorylation of			NULL	MOLT-3 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_14467_s_260	11839764	3 Therefore it is of interest that we observe (Fig.  6) that the interaction of EIIIA segment with alpha4beta1 in MOLT-3 cells increases phosphorylation of p44/42 MAP kinase.	bind
23800	1	7671	6	NULL	NULL	0	NULL	EIIIA segment	NULL		bind	NULL				alpha4beta1	NULL				NULL	MOLT-3 cells	0	NULL	NULL	NULL	gw60_jbiolchem_277_17_14467_s_260	11839764	3 Therefore it is of interest that we observe (Fig.  6) that the interaction of EIIIA segment with alpha4beta1 in MOLT-3 cells increases phosphorylation of p44/42 MAP kinase.	bind
23801	2	7671	6	10	NULL	0	NULL	statement 1			increases					p44/42 MAP kinase		phosphorylation of			NULL	MOLT-3 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_14467_s_260	11839764	3 Therefore it is of interest that we observe (Fig.  6) that the interaction of EIIIA segment with alpha4beta1 in MOLT-3 cells increases phosphorylation of p44/42 MAP kinase.	bind
30797	1	7672	5	13	NULL	NULL	NULL	NFkappaB	GP		regulates		may;;negatively			ISG	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_17_11678_s_162	16517601	3 Therefore, NFkappaB may negatively regulate ISG expression by directly or indirectly inhibiting the promoter binding of co-activators of ISG expression.	bind
30825	2	7672	5	13	NULL	NULL	NULL	co-activators	GP		bind					ISG	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_17_11678_s_162	16517601	3 Therefore, NFkappaB may negatively regulate ISG expression by directly or indirectly inhibiting the promoter binding of co-activators of ISG expression.	bind
30826	3	7672	5	13	NULL	NULL	NULL	NFkappaB	GP		inhibit		directly			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_17_11678_s_162	16517601	3 Therefore, NFkappaB may negatively regulate ISG expression by directly or indirectly inhibiting the promoter binding of co-activators of ISG expression.	bind
30827	4	7672	5	13	NULL	NULL	NULL	NFkappaB	GP		inhibit		indirectly			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_17_11678_s_162	16517601	3 Therefore, NFkappaB may negatively regulate ISG expression by directly or indirectly inhibiting the promoter binding of co-activators of ISG expression.	bind
30828	5	7672	5	13	NULL	NULL	NULL	statement 3	Process		is alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_17_11678_s_162	16517601	3 Therefore, NFkappaB may negatively regulate ISG expression by directly or indirectly inhibiting the promoter binding of co-activators of ISG expression.	bind
30829	6	7672	5	13	NULL	NULL	NULL	statement 3	Process		leads to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_17_11678_s_162	16517601	3 Therefore, NFkappaB may negatively regulate ISG expression by directly or indirectly inhibiting the promoter binding of co-activators of ISG expression.	bind
30830	7	7672	5	13	NULL	NULL	NULL	statement 4	Process		leads to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_17_11678_s_162	16517601	3 Therefore, NFkappaB may negatively regulate ISG expression by directly or indirectly inhibiting the promoter binding of co-activators of ISG expression.	bind
23802	1	7672	6	10	NULL	0	NULL	NFkappaB	NULL		 regulate	NULL	may;;negatively			ISG	NULL	expression of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_17_11678_s_162	16517601	3 Therefore, NFkappaB may negatively regulate ISG expression by directly or indirectly inhibiting the promoter binding of co-activators of ISG expression.	bind
23803	2	7672	6	NULL	NULL	0	NULL	co-activators	NULL		bind	NULL				ISG	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_17_11678_s_162	16517601	3 Therefore, NFkappaB may negatively regulate ISG expression by directly or indirectly inhibiting the promoter binding of co-activators of ISG expression.	bind
23804	3	7672	6	10	NULL	0	NULL	NF-kappaB	NULL		inhibits	NULL	directly			statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_17_11678_s_162	16517601	3 Therefore, NFkappaB may negatively regulate ISG expression by directly or indirectly inhibiting the promoter binding of co-activators of ISG expression.	bind
46643	4	7672	6	10	NULL	0	NULL	NFkappaB	NULL		inhibit	NULL	indirectly			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_17_11678_s_162	16517601	3 Therefore, NFkappaB may negatively regulate ISG expression by directly or indirectly inhibiting the promoter binding of co-activators of ISG expression.	bind
46644	5	7672	6	10	NULL	0	NULL	statement 3	NULL		is an alternative to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_17_11678_s_162	16517601	3 Therefore, NFkappaB may negatively regulate ISG expression by directly or indirectly inhibiting the promoter binding of co-activators of ISG expression.	bind
46645	6	7672	6	10	NULL	0	NULL	statement 3	NULL		leads to	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_17_11678_s_162	16517601	3 Therefore, NFkappaB may negatively regulate ISG expression by directly or indirectly inhibiting the promoter binding of co-activators of ISG expression.	bind
46646	7	7672	6	10	NULL	0	NULL	statement 4	NULL		leads to	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_17_11678_s_162	16517601	3 Therefore, NFkappaB may negatively regulate ISG expression by directly or indirectly inhibiting the promoter binding of co-activators of ISG expression.	bind
30798	1	7673	5	13	NULL	NULL	NULL	profilin	GP		bind					EVL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_46_36143_s_177	10945997	3 Therefore, we used profilin IIa to identify sequences through which profilin binds to EVL.	bind
23805	1	7673	6	NULL	NULL	0	NULL	profilin	NULL		bind	NULL				EVL	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_46_36143_s_177	10945997	3 Therefore, we used profilin IIa to identify sequences through which profilin binds to EVL.	bind
30799	1	7674	5	13	NULL	NULL	NULL	CRP	GP	native	bind					CD32	GP				NULL	on human neutrophils	NULL	NULL	NULL	NULL	gw70_circulationres_97_7_609_s_59	16195483	3 These authors have previously shown that native CRP binds to CD32, one of the Fc receptors, whereas mCRP binds to CD16, another Fc receptor isoform, on human neutrophils and exerting opposite function.	bind
30800	2	7674	5	13	NULL	NULL	NULL	CD32	GP		is a type of					Fc receptors	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_7_609_s_59	16195483	3 These authors have previously shown that native CRP binds to CD32, one of the Fc receptors, whereas mCRP binds to CD16, another Fc receptor isoform, on human neutrophils and exerting opposite function.	bind
30801	3	7674	5	13	NULL	NULL	NULL	mCRP	GP		bind					CD16	GP				NULL	on human neutrophils	NULL	NULL	NULL	NULL	gw70_circulationres_97_7_609_s_59	16195483	3 These authors have previously shown that native CRP binds to CD32, one of the Fc receptors, whereas mCRP binds to CD16, another Fc receptor isoform, on human neutrophils and exerting opposite function.	bind
30802	4	7674	5	13	NULL	NULL	NULL	CD16	GP		is a type of					Fc receptor isoform	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_7_609_s_59	16195483	3 These authors have previously shown that native CRP binds to CD32, one of the Fc receptors, whereas mCRP binds to CD16, another Fc receptor isoform, on human neutrophils and exerting opposite function.	bind
30803	5	7674	5	13	NULL	NULL	NULL	statement 1 	Process		exert opposite funtion to					statement 3	Process				NULL	human neutrophils	NULL	NULL	NULL	NULL	gw70_circulationres_97_7_609_s_59	16195483	3 These authors have previously shown that native CRP binds to CD32, one of the Fc receptors, whereas mCRP binds to CD16, another Fc receptor isoform, on human neutrophils and exerting opposite function.	bind
23806	1	7674	6	10	NULL	0	NULL	CRP	NULL	native	bind	NULL				CD32	NULL				NULL	human neutrophils	NULL	NULL	NULL	NULL	gw70_circulationres_97_7_609_s_59	16195483	3 These authors have previously shown that native CRP binds to CD32, one of the Fc receptors, whereas mCRP binds to CD16, another Fc receptor isoform, on human neutrophils and exerting opposite function.	bind
23807	2	7674	6	10	NULL	0	NULL	mCRP	NULL		bind	NULL				CD16	NULL				NULL	human neutrophils	NULL	NULL	NULL	NULL	gw70_circulationres_97_7_609_s_59	16195483	3 These authors have previously shown that native CRP binds to CD32, one of the Fc receptors, whereas mCRP binds to CD16, another Fc receptor isoform, on human neutrophils and exerting opposite function.	bind
46647	3	7674	6	10	NULL	0	NULL	CD32	NULL		is a type of	NULL				Fc receptors	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_7_609_s_59	16195483	3 These authors have previously shown that native CRP binds to CD32, one of the Fc receptors, whereas mCRP binds to CD16, another Fc receptor isoform, on human neutrophils and exerting opposite function.	bind
46648	4	7674	6	10	NULL	0	NULL	CD16	NULL		is a type of	NULL				Fc receptor isoform	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_7_609_s_59	16195483	3 These authors have previously shown that native CRP binds to CD32, one of the Fc receptors, whereas mCRP binds to CD16, another Fc receptor isoform, on human neutrophils and exerting opposite function.	bind
46649	5	7674	6	10	NULL	0	NULL	statement 1			exert opposite funtion to					statement 2					NULL	human neutrophils	NULL	NULL	NULL	NULL	gw70_circulationres_97_7_609_s_59	16195483	3 These authors have previously shown that native CRP binds to CD32, one of the Fc receptors, whereas mCRP binds to CD16, another Fc receptor isoform, on human neutrophils and exerting opposite function.	bind
30804	1	7675	5	13	NULL	NULL	NULL	alpha1	GP		bind			 A-domain		collagen IV	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12311_s_200	9139675	3 These techniques produced  K D values in the range of 1-5 nM, which is in good agreement with the figures obtained for alpha1 A-domain binding to collagen IV (6-34 nM;	bind
23808	1	7675	6	NULL	NULL	0	NULL	alpha1	NULL		bind	NULL		A domain		collagen IV	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_19_12311_s_200	9139675	3 These techniques produced  K D values in the range of 1-5 nM, which is in good agreement with the figures obtained for alpha1 A-domain binding to collagen IV (6-34 nM;	bind
30805	1	7676	5	13	NULL	NULL	NULL	NK-3	GP		bind					DNA	NucleicAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_40_25875_s_115	9748262	3 This effect may simply result from the enhancement of NK-3 DNA binding activity by HIPK2 that was seen in the  in vitro binding assays (Fig.  3).	bind
30806	2	7676	5	13	NULL	NULL	NULL	HIPK2	GP		enhances					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_40_25875_s_115	9748262	3 This effect may simply result from the enhancement of NK-3 DNA binding activity by HIPK2 that was seen in the  in vitro binding assays (Fig.  3).	bind
23809	1	7676	6	NULL	NULL	0	NULL	NK-3	NULL		bind	NULL				DNA	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_40_25875_s_115	9748262	3 This effect may simply result from the enhancement of NK-3 DNA binding activity by HIPK2 that was seen in the  in vitro binding assays (Fig.  3).	bind
23810	2	7676	6	10	NULL	0	NULL	HIPK2	NULL		enhances	NULL				statement 1	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_40_25875_s_115	9748262	3 This effect may simply result from the enhancement of NK-3 DNA binding activity by HIPK2 that was seen in the  in vitro binding assays (Fig.  3).	bind
30807	1	7677	5	13	NULL	NULL	NULL	PTB	GP		bind								UCUU motif within uridine-rich element region		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_21_22166_s_352	15010470	3 This feature does not allow testing by a mutational approach to know whether this downstream site is implicated in the repression of exon 9A9'', but it suggests a new model of regulation in which binding of PTB to the UCUU motif present within the uridine-rich element region could preclude CstF-64 binding.	bind
30808	2	7677	5	13	NULL	NULL	NULL	statement 1	Process		preclude					CstF-64	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_21_22166_s_352	15010470	3 This feature does not allow testing by a mutational approach to know whether this downstream site is implicated in the repression of exon 9A9'', but it suggests a new model of regulation in which binding of PTB to the UCUU motif present within the uridine-rich element region could preclude CstF-64 binding.	bind
23811	1	7677	6	10	NULL	0	NULL	PTB	NULL		bind	NULL					NULL		UCUU motif within uridine-rich element region		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_21_22166_s_352	15010470	3 This feature does not allow testing by a mutational approach to know whether this downstream site is implicated in the repression of exon 9A9'', but it suggests a new model of regulation in which binding of PTB to the UCUU motif present within the uridine-rich element region could preclude CstF-64 binding.	bind
46650	2	7677	6	10	NULL	0	NULL	statement 1	NULL		preclude	NULL				CstF-64	NULL	binding of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_21_22166_s_352	15010470	3 This feature does not allow testing by a mutational approach to know whether this downstream site is implicated in the repression of exon 9A9'', but it suggests a new model of regulation in which binding of PTB to the UCUU motif present within the uridine-rich element region could preclude CstF-64 binding.	bind
30809	1	7678	5	13	NULL	NULL	NULL	LRP	GP		is					LDL receptor-related protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1669_s_25	15178567	3 This implicates an endocytic step in selective uptake and prompted us to examine the role of the LDL receptor-related protein (LRP) 4 in selective uptake, particularly because the LRP binds to apolipoprotein E (apoE), lipoprotein lipase, and hepatic lipase, and these molecules have been shown to facilitate selective uptake.	bind
30810	2	7678	5	13	NULL	NULL	NULL	LRP	GP		bind					apoE	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1669_s_25	15178567	3 This implicates an endocytic step in selective uptake and prompted us to examine the role of the LDL receptor-related protein (LRP) 4 in selective uptake, particularly because the LRP binds to apolipoprotein E (apoE), lipoprotein lipase, and hepatic lipase, and these molecules have been shown to facilitate selective uptake.	bind
30811	3	7678	5	13	NULL	NULL	NULL	apoE	GP		is					apolipoprotein E	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1669_s_25	15178567	3 This implicates an endocytic step in selective uptake and prompted us to examine the role of the LDL receptor-related protein (LRP) 4 in selective uptake, particularly because the LRP binds to apolipoprotein E (apoE), lipoprotein lipase, and hepatic lipase, and these molecules have been shown to facilitate selective uptake.	bind
30812	4	7678	5	13	NULL	NULL	NULL	LRP	GP		bind					lipoprotein lipase	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1669_s_25	15178567	3 This implicates an endocytic step in selective uptake and prompted us to examine the role of the LDL receptor-related protein (LRP) 4 in selective uptake, particularly because the LRP binds to apolipoprotein E (apoE), lipoprotein lipase, and hepatic lipase, and these molecules have been shown to facilitate selective uptake.	bind
30813	5	7678	5	13	NULL	NULL	NULL	LRP	GP		bind					hepatic lipase	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1669_s_25	15178567	3 This implicates an endocytic step in selective uptake and prompted us to examine the role of the LDL receptor-related protein (LRP) 4 in selective uptake, particularly because the LRP binds to apolipoprotein E (apoE), lipoprotein lipase, and hepatic lipase, and these molecules have been shown to facilitate selective uptake.	bind
30814	6	7678	5	13	NULL	NULL	NULL	apoE	GP		facilitate					selective uptake	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1669_s_25	15178567	3 This implicates an endocytic step in selective uptake and prompted us to examine the role of the LDL receptor-related protein (LRP) 4 in selective uptake, particularly because the LRP binds to apolipoprotein E (apoE), lipoprotein lipase, and hepatic lipase, and these molecules have been shown to facilitate selective uptake.	bind
30815	7	7678	5	13	NULL	NULL	NULL	lipoprotein lipase	GP		facilitate					selective uptake	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1669_s_25	15178567	3 This implicates an endocytic step in selective uptake and prompted us to examine the role of the LDL receptor-related protein (LRP) 4 in selective uptake, particularly because the LRP binds to apolipoprotein E (apoE), lipoprotein lipase, and hepatic lipase, and these molecules have been shown to facilitate selective uptake.	bind
30816	8	7678	5	13	NULL	NULL	NULL	hepatic lipase	GP		facilitate					selective uptake	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1669_s_25	15178567	3 This implicates an endocytic step in selective uptake and prompted us to examine the role of the LDL receptor-related protein (LRP) 4 in selective uptake, particularly because the LRP binds to apolipoprotein E (apoE), lipoprotein lipase, and hepatic lipase, and these molecules have been shown to facilitate selective uptake.	bind
30817	9	7678	5	13	NULL	NULL	NULL	LRP	GP		plays a role in					selective uptake	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1669_s_25	15178567	3 This implicates an endocytic step in selective uptake and prompted us to examine the role of the LDL receptor-related protein (LRP) 4 in selective uptake, particularly because the LRP binds to apolipoprotein E (apoE), lipoprotein lipase, and hepatic lipase, and these molecules have been shown to facilitate selective uptake.	bind
23812	1	7678	6	NULL	NULL	0	NULL	LRP	NULL		is	NULL				LDL receptor-related protein	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1669_s_25	15178567	3 This implicates an endocytic step in selective uptake and prompted us to examine the role of the LDL receptor-related protein (LRP) 4 in selective uptake, particularly because the LRP binds to apolipoprotein E (apoE), lipoprotein lipase, and hepatic lipase, and these molecules have been shown to facilitate selective uptake.	bind
23813	2	7678	6	NULL	NULL	0	NULL	LRP	NULL		bind	NULL				apoE	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1669_s_25	15178567	3 This implicates an endocytic step in selective uptake and prompted us to examine the role of the LDL receptor-related protein (LRP) 4 in selective uptake, particularly because the LRP binds to apolipoprotein E (apoE), lipoprotein lipase, and hepatic lipase, and these molecules have been shown to facilitate selective uptake.	bind
23814	3	7678	6	NULL	NULL	0	NULL	apoE	NULL		is	NULL				apolipoprotein E	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1669_s_25	15178567	3 This implicates an endocytic step in selective uptake and prompted us to examine the role of the LDL receptor-related protein (LRP) 4 in selective uptake, particularly because the LRP binds to apolipoprotein E (apoE), lipoprotein lipase, and hepatic lipase, and these molecules have been shown to facilitate selective uptake.	bind
23815	4	7678	6	NULL	NULL	0	NULL	LRP	NULL		bind	NULL				lipoprotein lipase	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1669_s_25	15178567	3 This implicates an endocytic step in selective uptake and prompted us to examine the role of the LDL receptor-related protein (LRP) 4 in selective uptake, particularly because the LRP binds to apolipoprotein E (apoE), lipoprotein lipase, and hepatic lipase, and these molecules have been shown to facilitate selective uptake.	bind
23816	5	7678	6	NULL	NULL	0	NULL	LRP	NULL		bind	NULL				hepatic lipase	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1669_s_25	15178567	3 This implicates an endocytic step in selective uptake and prompted us to examine the role of the LDL receptor-related protein (LRP) 4 in selective uptake, particularly because the LRP binds to apolipoprotein E (apoE), lipoprotein lipase, and hepatic lipase, and these molecules have been shown to facilitate selective uptake.	bind
23817	6	7678	6	NULL	NULL	0	NULL	apoE	NULL		facilitate	NULL				selective uptake	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1669_s_25	15178567	3 This implicates an endocytic step in selective uptake and prompted us to examine the role of the LDL receptor-related protein (LRP) 4 in selective uptake, particularly because the LRP binds to apolipoprotein E (apoE), lipoprotein lipase, and hepatic lipase, and these molecules have been shown to facilitate selective uptake.	bind
23818	7	7678	6	NULL	NULL	0	NULL	lipoprotein lipase	NULL		facilitate	NULL				selective uptake	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1669_s_25	15178567	3 This implicates an endocytic step in selective uptake and prompted us to examine the role of the LDL receptor-related protein (LRP) 4 in selective uptake, particularly because the LRP binds to apolipoprotein E (apoE), lipoprotein lipase, and hepatic lipase, and these molecules have been shown to facilitate selective uptake.	bind
23819	8	7678	6	NULL	NULL	0	NULL	hepatic lipase	NULL		facilitate	NULL				selective uptake	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1669_s_25	15178567	3 This implicates an endocytic step in selective uptake and prompted us to examine the role of the LDL receptor-related protein (LRP) 4 in selective uptake, particularly because the LRP binds to apolipoprotein E (apoE), lipoprotein lipase, and hepatic lipase, and these molecules have been shown to facilitate selective uptake.	bind
46651	9	7678	6	10	NULL	0	NULL	LRP	NULL		plays a role in	NULL				selective uptake	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1669_s_25	15178567	3 This implicates an endocytic step in selective uptake and prompted us to examine the role of the LDL receptor-related protein (LRP) 4 in selective uptake, particularly because the LRP binds to apolipoprotein E (apoE), lipoprotein lipase, and hepatic lipase, and these molecules have been shown to facilitate selective uptake.	bind
30818	1	7679	5	13	NULL	NULL	NULL	fibrinogen	GP	bivalent	bind					(GP) IIb/IIa complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_17_2725_s_19	16246969	3 Thrombus forms as platelets aggregate via the binding of bivalent fibrinogen to the glycoprotein (GP) IIb/IIa complex.	bind
30819	2	7679	5	13	NULL	NULL	NULL	(GP) IIb/IIa complex	GP		is					glycoprotein IIb/IIa complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_17_2725_s_19	16246969	3 Thrombus forms as platelets aggregate via the binding of bivalent fibrinogen to the glycoprotein (GP) IIb/IIa complex.	bind
30820	3	7679	5	13	NULL	NULL	NULL	thrombus			forms					platelets aggregate	Cell				NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_17_2725_s_19	16246969	3 Thrombus forms as platelets aggregate via the binding of bivalent fibrinogen to the glycoprotein (GP) IIb/IIa complex.	bind
30821	4	7679	5	13	NULL	NULL	NULL	statement 3	Process		via					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_17_2725_s_19	16246969	3 Thrombus forms as platelets aggregate via the binding of bivalent fibrinogen to the glycoprotein (GP) IIb/IIa complex.	bind
23820	1	7679	6	NULL	NULL	0	NULL	fibrinogen	NULL	bivalent	bind	NULL				GP IIb/IIa complex	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_112_17_2725_s_19	16246969	3 Thrombus forms as platelets aggregate via the binding of bivalent fibrinogen to the glycoprotein (GP) IIb/IIa complex.	bind
23821	2	7679	6	NULL	NULL	0	NULL	GP	NULL		is	NULL				glycoprotein	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_112_17_2725_s_19	16246969	3 Thrombus forms as platelets aggregate via the binding of bivalent fibrinogen to the glycoprotein (GP) IIb/IIa complex.	bind
23822	3	7679	6	NULL	NULL	0	NULL	thrombus	NULL		forms as	NULL				platelets aggregate	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_112_17_2725_s_19	16246969	3 Thrombus forms as platelets aggregate via the binding of bivalent fibrinogen to the glycoprotein (GP) IIb/IIa complex.	bind
23823	4	7679	6	NULL	NULL	0	NULL	statement 3	NULL		occurs via	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_112_17_2725_s_19	16246969	3 Thrombus forms as platelets aggregate via the binding of bivalent fibrinogen to the glycoprotein (GP) IIb/IIa complex.	bind
30822	1	7680	5	13	NULL	NULL	NULL	IP6	GP		functions as		possibly			classic signaling molecule	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_47_36575_s_319	10960485	3 Thus, it remains possible that IP6 functions as a classic signaling molecule that directly binds an effector protein in the mRNA export machinery.	bind
30823	2	7680	5	13	NULL	NULL	NULL	IP6	GP		bind		directly			effector protein	GP				NULL	mRNA export machinery	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_47_36575_s_319	10960485	3 Thus, it remains possible that IP6 functions as a classic signaling molecule that directly binds an effector protein in the mRNA export machinery.	bind
23824	1	7680	6	NULL	NULL	0	NULL	IP6	NULL		bind	NULL	directly			effector protein	NULL				NULL	mRNA export machinery	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_47_36575_s_319	10960485	3 Thus, it remains possible that IP6 functions as a classic signaling molecule that directly binds an effector protein in the mRNA export machinery.	bind
46652	1	7680	6	10	NULL	0	NULL	IP6			functions as		possibly			 classic signaling molecule					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_47_36575_s_319	10960485	3 Thus, it remains possible that IP6 functions as a classic signaling molecule that directly binds an effector protein in the mRNA export machinery.	bind
30890	1	7681	5	13	NULL	NULL	NULL	cTnC	GP		bind					cTnI	GP		1-80		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_24_16681_s_41	10358006	3 To confirm the assignments for cTnC bound to cTnI-(1-80) and cTnI-(1-80)DD, 1H-15N NOESY-HSQC experiments with mixing times of 85 and 200 ms were performed at 800 MHz.	bind
30891	2	7681	5	13	NULL	NULL	NULL	cTnC	GP		bind					cTnI	GP		(1-80)DD		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_24_16681_s_41	10358006	3 To confirm the assignments for cTnC bound to cTnI-(1-80) and cTnI-(1-80)DD, 1H-15N NOESY-HSQC experiments with mixing times of 85 and 200 ms were performed at 800 MHz.	bind
23825	1	7681	6	NULL	NULL	0	NULL	cTnC	NULL		bind	NULL				cTnI	NULL		1-80		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_24_16681_s_41	10358006	3 To confirm the assignments for cTnC bound to cTnI-(1-80) and cTnI-(1-80)DD, 1H-15N NOESY-HSQC experiments with mixing times of 85 and 200 ms were performed at 800 MHz.	bind
23826	2	7681	6	NULL	NULL	0	NULL	cTnC	NULL		bind	NULL				cTnI	NULL		1-80 DD		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_24_16681_s_41	10358006	3 To confirm the assignments for cTnC bound to cTnI-(1-80) and cTnI-(1-80)DD, 1H-15N NOESY-HSQC experiments with mixing times of 85 and 200 ms were performed at 800 MHz.	bind
30892	1	7683	5	13	NULL	NULL	NULL	Ras	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39001_s_161	10967125	3 To rule out the possibility that the inhibition of apoptosis by hypoxic culture conditions, sodium butyrate treatment, or trichostatin A treatment were due to effects on Ras activity, Ras activity was analyzed by affinity binding to a Raf Ras-binding domain (RBD) peptide that only binds the activated (GTP-bound) form of Ras.	bind
30893	2	7683	5	13	NULL	NULL	NULL	Raf peptide	GP		bind			RBD		statement 1	GP	activated			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39001_s_161	10967125	3 To rule out the possibility that the inhibition of apoptosis by hypoxic culture conditions, sodium butyrate treatment, or trichostatin A treatment were due to effects on Ras activity, Ras activity was analyzed by affinity binding to a Raf Ras-binding domain (RBD) peptide that only binds the activated (GTP-bound) form of Ras.	bind
30894	3	7683	5	13	NULL	NULL	NULL	RBD	GP		is					Ras-binding domain	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39001_s_161	10967125	3 To rule out the possibility that the inhibition of apoptosis by hypoxic culture conditions, sodium butyrate treatment, or trichostatin A treatment were due to effects on Ras activity, Ras activity was analyzed by affinity binding to a Raf Ras-binding domain (RBD) peptide that only binds the activated (GTP-bound) form of Ras.	bind
23827	1	7683	6	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				Ras	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_50_39001_s_161	10967125	3 To rule out the possibility that the inhibition of apoptosis by hypoxic culture conditions, sodium butyrate treatment, or trichostatin A treatment were due to effects on Ras activity, Ras activity was analyzed by affinity binding to a Raf Ras-binding domain (RBD) peptide that only binds the activated (GTP-bound) form of Ras.	bind
23828	2	7683	6	NULL	NULL	0	NULL	Raf	NULL		bind	NULL	only	RBD		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_50_39001_s_161	10967125	3 To rule out the possibility that the inhibition of apoptosis by hypoxic culture conditions, sodium butyrate treatment, or trichostatin A treatment were due to effects on Ras activity, Ras activity was analyzed by affinity binding to a Raf Ras-binding domain (RBD) peptide that only binds the activated (GTP-bound) form of Ras.	bind
23829	3	7683	6	NULL	NULL	0	NULL	RBD	NULL		is	NULL				Ras-binding domain	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_50_39001_s_161	10967125	3 To rule out the possibility that the inhibition of apoptosis by hypoxic culture conditions, sodium butyrate treatment, or trichostatin A treatment were due to effects on Ras activity, Ras activity was analyzed by affinity binding to a Raf Ras-binding domain (RBD) peptide that only binds the activated (GTP-bound) form of Ras.	bind
30895	1	7684	5	13	NULL	NULL	NULL	VEGF	GP		bind					KDR/Flk-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_8_796_s_19	16151023	3 VEGF binds to its receptors KDR/Flk-1 to mediate its effect on angiogenesis in physiological conditions and in human atherosclerosis.	bind
30896	2	7684	5	13	NULL	NULL	NULL	statement 1	Process		mediates					angiogenesis	Process	effect on			NULL	in physiological conditions	NULL	NULL	NULL	NULL	gw70_circulationres_97_8_796_s_19	16151023	3 VEGF binds to its receptors KDR/Flk-1 to mediate its effect on angiogenesis in physiological conditions and in human atherosclerosis.	bind
30897	3	7684	5	13	NULL	NULL	NULL	statement 1	Process		mediates					angiogenesis	Process	effect on			NULL	in human atherosclerosis	NULL	NULL	NULL	NULL	gw70_circulationres_97_8_796_s_19	16151023	3 VEGF binds to its receptors KDR/Flk-1 to mediate its effect on angiogenesis in physiological conditions and in human atherosclerosis.	bind
23830	1	7684	6	NULL	NULL	0	NULL	VEGF	NULL		bind	NULL				KDR/Flk-1 receptor	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_8_796_s_19	16151023	3 VEGF binds to its receptors KDR/Flk-1 to mediate its effect on angiogenesis in physiological conditions and in human atherosclerosis.	bind
23831	2	7684	6	10	NULL	0	NULL	statement 1			mediates					angiogenesis		effect on			NULL	physiological conditions	NULL	NULL	NULL	NULL	gw70_circulationres_97_8_796_s_19	16151023	3 VEGF binds to its receptors KDR/Flk-1 to mediate its effect on angiogenesis in physiological conditions and in human atherosclerosis.	bind
23832	3	7684	6	10	NULL	0	NULL	statement 1			mediates					angiogenesis		effects on			NULL	human atherosclerosis	NULL	NULL	NULL	NULL	gw70_circulationres_97_8_796_s_19	16151023	3 VEGF binds to its receptors KDR/Flk-1 to mediate its effect on angiogenesis in physiological conditions and in human atherosclerosis.	bind
30898	1	7685	5	13	NULL	NULL	NULL	annexin V-FITC	GP		bind					platelets	Cell	PS-exposing			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_2_417_s_82	16339499	3 We determined platelet deposition and binding of annexin V-fluorescein isothiocyanate (FITC) to PS-exposing platelets after perfusion over a collagen-coated surface at a shear rate of 1000 s - 1.	bind
30899	2	7685	5	13	NULL	NULL	NULL	FITC	Chemical		is					fluorescein isothiocyanate	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_2_417_s_82	16339499	3 We determined platelet deposition and binding of annexin V-fluorescein isothiocyanate (FITC) to PS-exposing platelets after perfusion over a collagen-coated surface at a shear rate of 1000 s - 1.	bind
23834	1	7685	6	NULL	NULL	0	NULL	annexin V-fluorescein isothiocyanate	NULL		bind	NULL				platelets	NULL	PS-exposing			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_2_417_s_82	16339499	3 We determined platelet deposition and binding of annexin V-fluorescein isothiocyanate (FITC) to PS-exposing platelets after perfusion over a collagen-coated surface at a shear rate of 1000 s - 1.	bind
23835	2	7685	6	NULL	NULL	0	NULL	FITC	NULL		is	NULL				fluorescein isothiocyanate	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_2_417_s_82	16339499	3 We determined platelet deposition and binding of annexin V-fluorescein isothiocyanate (FITC) to PS-exposing platelets after perfusion over a collagen-coated surface at a shear rate of 1000 s - 1.	bind
30900	1	7686	5	13	NULL	NULL	NULL	LT	GP		is distinct from			GM1 binding site		LT	GP		LPS binding site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_8070_s_182	14660669	3 We previously demonstrated that the GM1 and LPS binding sites on LT are distinct ( ), and we wondered if a LPS binding site could be elucidated from the solved crystal structures of LT and CT ( ,   -  ).	bind
46730	1	7686	6	NULL	NULL	0	NULL	LT	NULL		is distinct from	NULL		GM1 binding site		LT	NULL		LPS binding site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_8070_s_182	14660669	3 We previously demonstrated that the GM1 and LPS binding sites on LT are distinct ( ), and we wondered if a LPS binding site could be elucidated from the solved crystal structures of LT and CT ( ,   -  ).	bind
30902	1	7687	5	13	NULL	NULL	NULL	COUP-TFII	GP		occupies					gAF1/PCK1	GP				NULL	in preadipocytes	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_32_30561_s_300	11399762	3 We propose that COUP-TFII occupies gAF1/PCK1 in preadipocytes and blocks activation of the PEPCK promoter via PPARgamma/RXR bound to PCK2.	bind
30903	2	7687	5	13	NULL	NULL	NULL	statement 1	Process		blocks					PEPCK	GP	activation of		promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_32_30561_s_300	11399762	3 We propose that COUP-TFII occupies gAF1/PCK1 in preadipocytes and blocks activation of the PEPCK promoter via PPARgamma/RXR bound to PCK2.	bind
30904	3	7687	5	13	NULL	NULL	NULL	PPARgamma/RXR	GP		bind					PCK2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_32_30561_s_300	11399762	3 We propose that COUP-TFII occupies gAF1/PCK1 in preadipocytes and blocks activation of the PEPCK promoter via PPARgamma/RXR bound to PCK2.	bind
30905	4	7687	5	13	NULL	NULL	NULL	statement 2	Process		via					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_32_30561_s_300	11399762	3 We propose that COUP-TFII occupies gAF1/PCK1 in preadipocytes and blocks activation of the PEPCK promoter via PPARgamma/RXR bound to PCK2.	bind
23911	1	7687	6	NULL	NULL	0	NULL	PPARgamma/RXR	NULL		bind	NULL				PCK2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_32_30561_s_300	11399762	3 We propose that COUP-TFII occupies gAF1/PCK1 in preadipocytes and blocks activation of the PEPCK promoter via PPARgamma/RXR bound to PCK2.	bind
23912	2	7687	6	NULL	NULL	0	NULL	COUP-TFII	NULL		occupies	NULL				gAF1/PCK1	NULL				NULL	preadipocytes	0	NULL	NULL	NULL	gw60_jbiolchem_276_32_30561_s_300	11399762	3 We propose that COUP-TFII occupies gAF1/PCK1 in preadipocytes and blocks activation of the PEPCK promoter via PPARgamma/RXR bound to PCK2.	bind
23913	3	7687	6	NULL	NULL	0	NULL	COUP-TFII	NULL		blocks	NULL				PEPCK	NULL	activation of		promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_32_30561_s_300	11399762	3 We propose that COUP-TFII occupies gAF1/PCK1 in preadipocytes and blocks activation of the PEPCK promoter via PPARgamma/RXR bound to PCK2.	bind
23914	4	7687	6	NULL	NULL	0	NULL	statement 3	NULL		occurs via	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_32_30561_s_300	11399762	3 We propose that COUP-TFII occupies gAF1/PCK1 in preadipocytes and blocks activation of the PEPCK promoter via PPARgamma/RXR bound to PCK2.	bind
30907	1	7688	5	13	NULL	NULL	NULL	His6-Rvs167	GP	recombinant	bind					GST-Sla1	GP		1 - 420		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_16_16017_s_204	14761940	3 We were unable to test direct binding of Rvs167 to Sla1 720 - 1240 because GST-Sla1 720 - 1240 was not stably expressed in  E. coli; however, recombinant His6-Rvs167 bound to GST-Sla1 1 - 420 and weakly to GST-Sla1 420 - 720 ( Fig. 5 B), indicating that Rvs167 binds to Sla1 directly, perhaps via multiple sites.	bind
30908	2	7688	5	13	NULL	NULL	NULL	His6-Rvs167	GP	recombinant	bind		weakly			GST-Sla1	GP		420 - 720		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_16_16017_s_204	14761940	3 We were unable to test direct binding of Rvs167 to Sla1 720 - 1240 because GST-Sla1 720 - 1240 was not stably expressed in  E. coli; however, recombinant His6-Rvs167 bound to GST-Sla1 1 - 420 and weakly to GST-Sla1 420 - 720 ( Fig. 5 B), indicating that Rvs167 binds to Sla1 directly, perhaps via multiple sites.	bind
30909	3	7688	5	13	NULL	NULL	NULL	Rvs167	GP		bind		directly			Sla1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_16_16017_s_204	14761940	3 We were unable to test direct binding of Rvs167 to Sla1 720 - 1240 because GST-Sla1 720 - 1240 was not stably expressed in  E. coli; however, recombinant His6-Rvs167 bound to GST-Sla1 1 - 420 and weakly to GST-Sla1 420 - 720 ( Fig. 5 B), indicating that Rvs167 binds to Sla1 directly, perhaps via multiple sites.	bind
30910	4	7688	5	13	NULL	NULL	NULL	statement 3	Process		via					multiple sites	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_16_16017_s_204	14761940	3 We were unable to test direct binding of Rvs167 to Sla1 720 - 1240 because GST-Sla1 720 - 1240 was not stably expressed in  E. coli; however, recombinant His6-Rvs167 bound to GST-Sla1 1 - 420 and weakly to GST-Sla1 420 - 720 ( Fig. 5 B), indicating that Rvs167 binds to Sla1 directly, perhaps via multiple sites.	bind
23915	1	7688	6	NULL	NULL	0	NULL	His6-Rvs167	NULL	recombinant	bind	NULL				GST-Sla1	NULL		1-420		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_16017_s_204	14761940	3 We were unable to test direct binding of Rvs167 to Sla1 720 - 1240 because GST-Sla1 720 - 1240 was not stably expressed in  E. coli; however, recombinant His6-Rvs167 bound to GST-Sla1 1 - 420 and weakly to GST-Sla1 420 - 720 ( Fig. 5 B), indicating that Rvs167 binds to Sla1 directly, perhaps via multiple sites.	bind
23916	2	7688	6	NULL	NULL	0	NULL	His6-Rvs167	NULL	recombinant	bind	NULL	weakly			GST-Sla1	NULL		420-720		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_16017_s_204	14761940	3 We were unable to test direct binding of Rvs167 to Sla1 720 - 1240 because GST-Sla1 720 - 1240 was not stably expressed in  E. coli; however, recombinant His6-Rvs167 bound to GST-Sla1 1 - 420 and weakly to GST-Sla1 420 - 720 ( Fig. 5 B), indicating that Rvs167 binds to Sla1 directly, perhaps via multiple sites.	bind
46731	3	7688	6	10	NULL	0	NULL	Rvs167 	NULL		bind	NULL	directly			Sla1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_16017_s_204	14761940	3 We were unable to test direct binding of Rvs167 to Sla1 720 - 1240 because GST-Sla1 720 - 1240 was not stably expressed in  E. coli; however, recombinant His6-Rvs167 bound to GST-Sla1 1 - 420 and weakly to GST-Sla1 420 - 720 ( Fig. 5 B), indicating that Rvs167 binds to Sla1 directly, perhaps via multiple sites.	bind
46732	4	7688	6	10	NULL	0	NULL	statement 3	NULL		via	NULL				multiple sites	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_16017_s_204	14761940	3 We were unable to test direct binding of Rvs167 to Sla1 720 - 1240 because GST-Sla1 720 - 1240 was not stably expressed in  E. coli; however, recombinant His6-Rvs167 bound to GST-Sla1 1 - 420 and weakly to GST-Sla1 420 - 720 ( Fig. 5 B), indicating that Rvs167 binds to Sla1 directly, perhaps via multiple sites.	bind
30911	1	7689	5	13	NULL	NULL	NULL	IdceA unit	GP	2- O-sulfated	is a part of					3- O -sulfotransferase	GP		substrate recognition site 		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_30_18770_s_250	9668050	3 While this conclusion is probably correct, it is recalled that a 2- O-sulfated IdceA unit was identified as part of the substrate recognition site for the 3- O -sulfotransferaseinvolved in the biosynthesis of the antithrombin-binding region ( 52); a polysaccharide devoid of HexA 2- O-sulfate groups thus will probably lack GlcN 3- O-sulfate substituents.	bind
30912	2	7689	5	13	NULL	NULL	NULL	3- O -sulfotransferase	GP		is involved in							biosynthesis of	antithrombin-binding region		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_30_18770_s_250	9668050	3 While this conclusion is probably correct, it is recalled that a 2- O-sulfated IdceA unit was identified as part of the substrate recognition site for the 3- O -sulfotransferaseinvolved in the biosynthesis of the antithrombin-binding region ( 52); a polysaccharide devoid of HexA 2- O-sulfate groups thus will probably lack GlcN 3- O-sulfate substituents.	bind
30913	3	7689	5	13	NULL	NULL	NULL	polysaccharide	Chemical		devoid of					HexA 2- O-sulfate groups	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_30_18770_s_250	9668050	3 While this conclusion is probably correct, it is recalled that a 2- O-sulfated IdceA unit was identified as part of the substrate recognition site for the 3- O -sulfotransferaseinvolved in the biosynthesis of the antithrombin-binding region ( 52); a polysaccharide devoid of HexA 2- O-sulfate groups thus will probably lack GlcN 3- O-sulfate substituents.	bind
46733	4	7689	5	13	NULL	NULL	NULL	statement 3	Chemical		lack		probably			GlcN 3- O-sulfate substituents	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_30_18770_s_250	9668050	3 While this conclusion is probably correct, it is recalled that a 2- O-sulfated IdceA unit was identified as part of the substrate recognition site for the 3- O -sulfotransferaseinvolved in the biosynthesis of the antithrombin-binding region ( 52); a polysaccharide devoid of HexA 2- O-sulfate groups thus will probably lack GlcN 3- O-sulfate substituents.	bind
24473	1	7689	6	10	NULL	0	NULL	IdceA unit		2- O-sulfated	is part of the 					3- O -sulfotransferase			substrate recognition site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_30_18770_s_250	9668050	3 While this conclusion is probably correct, it is recalled that a 2- O-sulfated IdceA unit was identified as part of the substrate recognition site for the 3- O -sulfotransferaseinvolved in the biosynthesis of the antithrombin-binding region ( 52); a polysaccharide devoid of HexA 2- O-sulfate groups thus will probably lack GlcN 3- O-sulfate substituents.	bind
24474	2	7689	6	10	NULL	0	NULL	3-O-sulfotransferase	NULL		is involved in	NULL					NULL	biosynthesis of	antithrombin-binding region		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_30_18770_s_250	9668050	3 While this conclusion is probably correct, it is recalled that a 2- O-sulfated IdceA unit was identified as part of the substrate recognition site for the 3- O -sulfotransferaseinvolved in the biosynthesis of the antithrombin-binding region ( 52); a polysaccharide devoid of HexA 2- O-sulfate groups thus will probably lack GlcN 3- O-sulfate substituents.	bind
24475	3	7689	6	10	NULL	0	NULL	polysaccharide	NULL		devoid of	NULL				HexA 2- O-sulfate group	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_30_18770_s_250	9668050	3 While this conclusion is probably correct, it is recalled that a 2- O-sulfated IdceA unit was identified as part of the substrate recognition site for the 3- O -sulfotransferaseinvolved in the biosynthesis of the antithrombin-binding region ( 52); a polysaccharide devoid of HexA 2- O-sulfate groups thus will probably lack GlcN 3- O-sulfate substituents.	bind
46734	4	7689	6	10	NULL	0	NULL	statement 3	NULL		lack	NULL	probably			GlcN 3- O-sulfate substituents	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_30_18770_s_250	9668050	3 While this conclusion is probably correct, it is recalled that a 2- O-sulfated IdceA unit was identified as part of the substrate recognition site for the 3- O -sulfotransferaseinvolved in the biosynthesis of the antithrombin-binding region ( 52); a polysaccharide devoid of HexA 2- O-sulfate groups thus will probably lack GlcN 3- O-sulfate substituents.	bind
30914	1	7690	5	13	NULL	NULL	NULL	3' processing	Process		is dependent on					snoRNP protein	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5415_s_236	10891482	3' processing appears to be dependent on snoRNP protein binding, but assembly with the mature snoRNP proteins may be incompatible with assembly of a functional spliceosome.	bind
30916	2	7690	5	13	NULL	NULL	NULL	snoRNP proteins	GP	assembly with;;mature	incompatible with		may be			functional spliceosome	CellComponent	assembly of a 			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5415_s_236	10891482	3' processing appears to be dependent on snoRNP protein binding, but assembly with the mature snoRNP proteins may be incompatible with assembly of a functional spliceosome.	bind
24546	1	7690	6	10	NULL	0	NULL	3' processing			is dependent on					snoRNP protein 		binding of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5415_s_236	10891482	3' processing appears to be dependent on snoRNP protein binding, but assembly with the mature snoRNP proteins may be incompatible with assembly of a functional spliceosome.	bind
24547	2	7690	6	10	NULL	0	NULL	snoRNP proteins		assembly with;;mature 	is incompatible with		may			functional spliceosome		assembly of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5415_s_236	10891482	3' processing appears to be dependent on snoRNP protein binding, but assembly with the mature snoRNP proteins may be incompatible with assembly of a functional spliceosome.	bind
30921	1	7691	5	13	NULL	NULL	NULL	TCDD	GP		bind					AhR	GP	rat liver			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_55_4_716_s_172	10101030	3''-OMe-4''-NO2-flavone is a competitive inhibitor of TCDD binding to rat liver AhR.	bind
30923	2	7691	5	13	NULL	NULL	NULL	3''-OMe-4''-NO2-flavone	Chemical		inhibits		competitively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_55_4_716_s_172	10101030	3''-OMe-4''-NO2-flavone is a competitive inhibitor of TCDD binding to rat liver AhR.	bind
23917	1	7691	6	NULL	NULL	0	NULL	TCDD	NULL		bind	NULL				AhR	NULL	rat liver			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_55_4_716_s_172	10101030	3''-OMe-4''-NO2-flavone is a competitive inhibitor of TCDD binding to rat liver AhR.	bind
23918	2	7691	6	NULL	NULL	0	NULL	3''-OMe-4''-NO2-flavone	NULL		inhibits	NULL	competitively			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_55_4_716_s_172	10101030	3''-OMe-4''-NO2-flavone is a competitive inhibitor of TCDD binding to rat liver AhR.	bind
30931	1	7692	5	13	NULL	NULL	NULL	CDK2	GP		bind		stably			PCNA	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_faseb-j_20_7_16675840_s_7	16675840	3)  At DNA replication sites, PCNA function may be envisaged with a model  of "`dynamic hand-off"` of interacting partners that rapidly and transiently  exchange in a mutually exclusive manner, while cyclin-dependent kinase  (Cdk) 2 (CDK2) is stably bound to PCNA.	bind
30932	2	7692	5	13	NULL	NULL	NULL	CDK2	GP		is					cyclin-dependent kinase 2	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_faseb-j_20_7_16675840_s_7	16675840	3)  At DNA replication sites, PCNA function may be envisaged with a model  of "`dynamic hand-off"` of interacting partners that rapidly and transiently  exchange in a mutually exclusive manner, while cyclin-dependent kinase  (Cdk) 2 (CDK2) is stably bound to PCNA.	bind
23919	1	7692	6	NULL	NULL	0	NULL	cdk2	NULL		bind	NULL	stably			PCNA	NULL				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_faseb-j_20_7_16675840_s_7	16675840	3)  At DNA replication sites, PCNA function may be envisaged with a model  of "`dynamic hand-off"` of interacting partners that rapidly and transiently  exchange in a mutually exclusive manner, while cyclin-dependent kinase  (Cdk) 2 (CDK2) is stably bound to PCNA.	bind
23920	2	7692	6	NULL	NULL	0	NULL	cdk2	NULL		is	NULL				cyclin-dependent kinase	NULL				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_faseb-j_20_7_16675840_s_7	16675840	3)  At DNA replication sites, PCNA function may be envisaged with a model  of "`dynamic hand-off"` of interacting partners that rapidly and transiently  exchange in a mutually exclusive manner, while cyclin-dependent kinase  (Cdk) 2 (CDK2) is stably bound to PCNA.	bind
30933	1	7693	5	13	NULL	NULL	NULL	180 kDa protein	GP		bind					PCNA	GP			E2F-like site	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_2_1218_s_252	8557653	3)  Results from a UV cross-linking experiment indicate that a protein of  180 kDa binds to the PCNA E2F-like site.	bind
23921	1	7693	6	NULL	NULL	0	NULL	protein 180kDa	NULL		bind	NULL				PCNA	NULL			E2F-like site	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_2_1218_s_252	8557653	3)  Results from a UV cross-linking experiment indicate that a protein of  180 kDa binds to the PCNA E2F-like site.	bind
30936	1	7694	5	13	NULL	NULL	NULL	troponin	GP		bind					tropomyosin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_43_25455_s_187	7592713	3)  There is a direct relationship between the strength of troponin binding  to tropomyosin (as the amino-terminal region of TnT is progressively  deleted or included), and the ability of troponin to enhance  tropomyosin-actin binding.	bind
30938	2	7694	5	13	NULL	NULL	NULL	tropomyosin	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_43_25455_s_187	7592713	3)  There is a direct relationship between the strength of troponin binding  to tropomyosin (as the amino-terminal region of TnT is progressively  deleted or included), and the ability of troponin to enhance  tropomyosin-actin binding.	bind
30939	3	7694	5	13	NULL	NULL	NULL	troponin	GP		enhance					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_43_25455_s_187	7592713	3)  There is a direct relationship between the strength of troponin binding  to tropomyosin (as the amino-terminal region of TnT is progressively  deleted or included), and the ability of troponin to enhance  tropomyosin-actin binding.	bind
30940	4	7694	5	13	NULL	NULL	NULL	statement 1	Process	strength of	is related to		directly			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_43_25455_s_187	7592713	3)  There is a direct relationship between the strength of troponin binding  to tropomyosin (as the amino-terminal region of TnT is progressively  deleted or included), and the ability of troponin to enhance  tropomyosin-actin binding.	bind
23922	1	7694	6	NULL	NULL	0	NULL	troponin	NULL		bind	NULL				tropomyosin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_43_25455_s_187	7592713	3)  There is a direct relationship between the strength of troponin binding  to tropomyosin (as the amino-terminal region of TnT is progressively  deleted or included), and the ability of troponin to enhance  tropomyosin-actin binding.	bind
23923	2	7694	6	NULL	NULL	0	NULL	tropomyosin	NULL		bind	NULL				actin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_43_25455_s_187	7592713	3)  There is a direct relationship between the strength of troponin binding  to tropomyosin (as the amino-terminal region of TnT is progressively  deleted or included), and the ability of troponin to enhance  tropomyosin-actin binding.	bind
23924	3	7694	6	NULL	NULL	0	NULL	troponin	NULL		enhance	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_43_25455_s_187	7592713	3)  There is a direct relationship between the strength of troponin binding  to tropomyosin (as the amino-terminal region of TnT is progressively  deleted or included), and the ability of troponin to enhance  tropomyosin-actin binding.	bind
46735	4	7694	6	10	NULL	0	NULL	statement 1	NULL	strength of	related to	NULL	directly			statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_43_25455_s_187	7592713	3)  There is a direct relationship between the strength of troponin binding  to tropomyosin (as the amino-terminal region of TnT is progressively  deleted or included), and the ability of troponin to enhance  tropomyosin-actin binding.	bind
30942	1	7695	5	13	NULL	NULL	NULL	STAT6	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_48_38095_s_260	10982806	3) A mutation in the DNA-binding domain of STAT6 selectively influenced STAT6 DNA binding preference leading to a blockade in IL-4-driven transcription.	bind
30944	2	7695	5	13	NULL	NULL	NULL	STAT6 	GP	mutant	influence		selectively	DNA-binding domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_48_38095_s_260	10982806	3) A mutation in the DNA-binding domain of STAT6 selectively influenced STAT6 DNA binding preference leading to a blockade in IL-4-driven transcription.	bind
30945	4	7695	5	13	NULL	NULL	NULL	statement 2	Process		blocks					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_48_38095_s_260	10982806	3) A mutation in the DNA-binding domain of STAT6 selectively influenced STAT6 DNA binding preference leading to a blockade in IL-4-driven transcription.	bind
46736	3	7695	5	13	NULL	NULL	NULL	IL-4	GP		drives					transcription	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_48_38095_s_260	10982806	3) A mutation in the DNA-binding domain of STAT6 selectively influenced STAT6 DNA binding preference leading to a blockade in IL-4-driven transcription.	bind
23925	1	7695	6	NULL	NULL	0	NULL	STAT6	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_48_38095_s_260	10982806	3) A mutation in the DNA-binding domain of STAT6 selectively influenced STAT6 DNA binding preference leading to a blockade in IL-4-driven transcription.	bind
23926	2	7695	6	NULL	NULL	0	NULL	STAT6	NULL	mutant	influence 	NULL	selectively	DNA binding domain 		statement 1	NULL	preference of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_48_38095_s_260	10982806	3) A mutation in the DNA-binding domain of STAT6 selectively influenced STAT6 DNA binding preference leading to a blockade in IL-4-driven transcription.	bind
23927	3	7695	6	10	NULL	0	NULL	IL-4	NULL		drives	NULL				transcription	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_48_38095_s_260	10982806	3) A mutation in the DNA-binding domain of STAT6 selectively influenced STAT6 DNA binding preference leading to a blockade in IL-4-driven transcription.	bind
46737	4	7695	6	10	NULL	0	NULL	statement 2	NULL		blocks	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_48_38095_s_260	10982806	3) A mutation in the DNA-binding domain of STAT6 selectively influenced STAT6 DNA binding preference leading to a blockade in IL-4-driven transcription.	bind
30948	1	7696	5	13	NULL	NULL	NULL	AGGTCA	GP		is a type of					single core motif	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_16_10565_s_184	9099702	3) A single core motif, AGGTCA, preceded by TCA (defined as 1/2-RTRE) is sufficient for RTR binding; however, the apparent affinity of RTR for 1/2-RTRE is significantly lower than that for conRTRE.	bind
30949	2	7696	5	NULL	NULL	0	NULL		NULL		is preceded by	NULL			AGGTCA		NULL			TCA	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_16_10565_s_184	9099702	3) A single core motif, AGGTCA, preceded by TCA (defined as 1/2-RTRE) is sufficient for RTR binding; however, the apparent affinity of RTR for 1/2-RTRE is significantly lower than that for conRTRE.	bind
30950	3	7696	5	13	NULL	NULL	NULL	AGGTCA	GP		is defined as					1/2-RTRE	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_16_10565_s_184	9099702	3) A single core motif, AGGTCA, preceded by TCA (defined as 1/2-RTRE) is sufficient for RTR binding; however, the apparent affinity of RTR for 1/2-RTRE is significantly lower than that for conRTRE.	bind
30951	4	7696	5	13	NULL	NULL	NULL				is sufficient for				AGGTCA	RTR	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_16_10565_s_184	9099702	3) A single core motif, AGGTCA, preceded by TCA (defined as 1/2-RTRE) is sufficient for RTR binding; however, the apparent affinity of RTR for 1/2-RTRE is significantly lower than that for conRTRE.	bind
30952	5	7696	5	13	NULL	NULL	NULL	RTR	GP		has affinity for									1/2-RTRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_16_10565_s_184	9099702	3) A single core motif, AGGTCA, preceded by TCA (defined as 1/2-RTRE) is sufficient for RTR binding; however, the apparent affinity of RTR for 1/2-RTRE is significantly lower than that for conRTRE.	bind
30953	6	7696	5	13	NULL	NULL	NULL	RTR	GP		has affinity for									conRTRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_16_10565_s_184	9099702	3) A single core motif, AGGTCA, preceded by TCA (defined as 1/2-RTRE) is sufficient for RTR binding; however, the apparent affinity of RTR for 1/2-RTRE is significantly lower than that for conRTRE.	bind
30958	7	7696	5	13	NULL	NULL	NULL	statement 5	Process	affinity of	lower than		significantly			statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_16_10565_s_184	9099702	3) A single core motif, AGGTCA, preceded by TCA (defined as 1/2-RTRE) is sufficient for RTR binding; however, the apparent affinity of RTR for 1/2-RTRE is significantly lower than that for conRTRE.	bind
24548	1	7696	6	NULL	NULL	0	NULL	RTR	NULL		has affinity for	NULL					NULL			1/2-RTRE	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10565_s_184	9099702	3) A single core motif, AGGTCA, preceded by TCA (defined as 1/2-RTRE) is sufficient for RTR binding; however, the apparent affinity of RTR for 1/2-RTRE is significantly lower than that for conRTRE.	bind
24549	2	7696	6	NULL	NULL	0	NULL	RTR	NULL		has affinity for	NULL					NULL			conRTRE	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10565_s_184	9099702	3) A single core motif, AGGTCA, preceded by TCA (defined as 1/2-RTRE) is sufficient for RTR binding; however, the apparent affinity of RTR for 1/2-RTRE is significantly lower than that for conRTRE.	bind
24550	3	7696	6	NULL	NULL	0	NULL	statement 1	NULL		is lower than	NULL	significantly			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10565_s_184	9099702	3) A single core motif, AGGTCA, preceded by TCA (defined as 1/2-RTRE) is sufficient for RTR binding; however, the apparent affinity of RTR for 1/2-RTRE is significantly lower than that for conRTRE.	bind
24551	4	7696	6	10	NULL	0	NULL	AGGTCA			is a type of					single core motif					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_16_10565_s_184	9099702	3) A single core motif, AGGTCA, preceded by TCA (defined as 1/2-RTRE) is sufficient for RTR binding; however, the apparent affinity of RTR for 1/2-RTRE is significantly lower than that for conRTRE.	bind
46890	5	7696	6	NULL	NULL	0	NULL		NULL		is sufficient for	NULL			1/2-RTRE	RTR	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10565_s_184	9099702	3) A single core motif, AGGTCA, preceded by TCA (defined as 1/2-RTRE) is sufficient for RTR binding; however, the apparent affinity of RTR for 1/2-RTRE is significantly lower than that for conRTRE.	bind
55542	6	7696	6	10	NULL	0	NULL				is preceded by				AGGTCA					TCA	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10565_s_184	9099702	3) A single core motif, AGGTCA, preceded by TCA (defined as 1/2-RTRE) is sufficient for RTR binding; however, the apparent affinity of RTR for 1/2-RTRE is significantly lower than that for conRTRE.	bind
55543	7	7696	6	10	NULL	0	NULL	AGGTCA			is defined as					1/2-RTRE					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10565_s_184	9099702	3) A single core motif, AGGTCA, preceded by TCA (defined as 1/2-RTRE) is sufficient for RTR binding; however, the apparent affinity of RTR for 1/2-RTRE is significantly lower than that for conRTRE.	bind
30960	1	7697	5	13	NULL	NULL	NULL				is a type of			Pro424 - Gly440		synthetic peptide	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_36_34395_s_229	12816955	3) a synthetic  peptide (Pro424 - Gly440) corresponding to sequences  within W4, but not its scrambled control, bound C3bi directly with a   Kd of 20 muM  ( Fig. 5 A).	bind
30961	2	7697	5	13	NULL	NULL	NULL				corresponds to			Pro424 - Gly440		W4	GP	sequences within			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_36_34395_s_229	12816955	3) a synthetic  peptide (Pro424 - Gly440) corresponding to sequences  within W4, but not its scrambled control, bound C3bi directly with a   Kd of 20 muM  ( Fig. 5 A).	bind
30963	3	7697	5	13	NULL	NULL	NULL				bind		directly	Pro424 - Gly440		C3bi	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_36_34395_s_229	12816955	3) a synthetic  peptide (Pro424 - Gly440) corresponding to sequences  within W4, but not its scrambled control, bound C3bi directly with a   Kd of 20 muM  ( Fig. 5 A).	bind
23928	1	7697	6	10	NULL	0	NULL		NULL		bind	NULL	directly	Pro424-Gly440		C3bi	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_36_34395_s_229	12816955	3) a synthetic  peptide (Pro424 - Gly440) corresponding to sequences  within W4, but not its scrambled control, bound C3bi directly with a   Kd of 20 muM  ( Fig. 5 A).	bind
46738	2	7697	6	10	NULL	0	NULL		NULL		is a type of	NULL		Pro424 - Gly440		synthetic peptide	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_36_34395_s_229	12816955	3) a synthetic  peptide (Pro424 - Gly440) corresponding to sequences  within W4, but not its scrambled control, bound C3bi directly with a   Kd of 20 muM  ( Fig. 5 A).	bind
46739	3	7697	6	10	NULL	0	NULL		NULL		corresponds to	NULL		Pro424 - Gly440		W4	NULL	sequences within			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_36_34395_s_229	12816955	3) a synthetic  peptide (Pro424 - Gly440) corresponding to sequences  within W4, but not its scrambled control, bound C3bi directly with a   Kd of 20 muM  ( Fig. 5 A).	bind
30964	1	7698	5	13	NULL	NULL	NULL	alpha beta	GP		bind					iC3b	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_43_25866_s_149	7592772	3) Alanine substitution of Asp ,  Tyr , or deletion of residues  Phe -Tyr   (delta246-252)  abolished the binding of alpha beta   to iC3b as  well as the recognition of the function blocking anti-alpha   antibody 3H5.	bind
30965	2	7698	5	13	NULL	NULL	NULL	statement 8	Process		abolishes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_43_25866_s_149	7592772	3) Alanine substitution of Asp ,  Tyr , or deletion of residues  Phe -Tyr   (delta246-252)  abolished the binding of alpha beta   to iC3b as  well as the recognition of the function blocking anti-alpha   antibody 3H5.	bind
30966	3	7698	5	13	NULL	NULL	NULL	statement 9	Process		abolishes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_43_25866_s_149	7592772	3) Alanine substitution of Asp ,  Tyr , or deletion of residues  Phe -Tyr   (delta246-252)  abolished the binding of alpha beta   to iC3b as  well as the recognition of the function blocking anti-alpha   antibody 3H5.	bind
30968	4	7698	5	13	NULL	NULL	NULL			deletion of	abolishes			Phe -Tyr (delta246-252)		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_43_25866_s_149	7592772	3) Alanine substitution of Asp ,  Tyr , or deletion of residues  Phe -Tyr   (delta246-252)  abolished the binding of alpha beta   to iC3b as  well as the recognition of the function blocking anti-alpha   antibody 3H5.	bind
30971	5	7698	5	13	NULL	NULL	NULL	statement 8	Process		blocks					anti-alpha antibody 3H5	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_43_25866_s_149	7592772	3) Alanine substitution of Asp ,  Tyr , or deletion of residues  Phe -Tyr   (delta246-252)  abolished the binding of alpha beta   to iC3b as  well as the recognition of the function blocking anti-alpha   antibody 3H5.	bind
30973	6	7698	5	13	NULL	NULL	NULL	statement 9	Process		block					anti-alpha antibody 3H5	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_43_25866_s_149	7592772	3) Alanine substitution of Asp ,  Tyr , or deletion of residues  Phe -Tyr   (delta246-252)  abolished the binding of alpha beta   to iC3b as  well as the recognition of the function blocking anti-alpha   antibody 3H5.	bind
30974	7	7698	5	13	NULL	NULL	NULL			deletion of	block			Phe -Tyr (delta246-252)		anti-alpha antibody 3H5	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_43_25866_s_149	7592772	3) Alanine substitution of Asp ,  Tyr , or deletion of residues  Phe -Tyr   (delta246-252)  abolished the binding of alpha beta   to iC3b as  well as the recognition of the function blocking anti-alpha   antibody 3H5.	bind
55535	8	7698	5	10	NULL	0	NULL				is substituted for			Asp					alanine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_43_25866_s_149	7592772	3) Alanine substitution of Asp ,  Tyr , or deletion of residues  Phe -Tyr   (delta246-252)  abolished the binding of alpha beta   to iC3b as  well as the recognition of the function blocking anti-alpha   antibody 3H5.	bind
55536	9	7698	5	10	NULL	0	NULL				is substituted for			Tyr					alanine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_43_25866_s_149	7592772	3) Alanine substitution of Asp ,  Tyr , or deletion of residues  Phe -Tyr   (delta246-252)  abolished the binding of alpha beta   to iC3b as  well as the recognition of the function blocking anti-alpha   antibody 3H5.	bind
23929	1	7698	6	NULL	NULL	0	NULL	alpha beta	NULL		bind	NULL				iC3b	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_43_25866_s_149	7592772	3) Alanine substitution of Asp ,  Tyr , or deletion of residues  Phe -Tyr   (delta246-252)  abolished the binding of alpha beta   to iC3b as  well as the recognition of the function blocking anti-alpha   antibody 3H5.	bind
23930	2	7698	6	NULL	NULL	0	NULL		NULL	deletion of	abolishes	NULL		residues Phe -Tyr (delta246-252)		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_43_25866_s_149	7592772	3) Alanine substitution of Asp ,  Tyr , or deletion of residues  Phe -Tyr   (delta246-252)  abolished the binding of alpha beta   to iC3b as  well as the recognition of the function blocking anti-alpha   antibody 3H5.	bind
24947	3	7698	6	10	NULL	0	NULL	statement 5			abolishes					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_43_25866_s_149	7592772	3) Alanine substitution of Asp ,  Tyr , or deletion of residues  Phe -Tyr   (delta246-252)  abolished the binding of alpha beta   to iC3b as  well as the recognition of the function blocking anti-alpha   antibody 3H5.	bind
24948	4	7698	6	10	NULL	0	NULL	statement 6			abolishes					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_43_25866_s_149	7592772	3) Alanine substitution of Asp ,  Tyr , or deletion of residues  Phe -Tyr   (delta246-252)  abolished the binding of alpha beta   to iC3b as  well as the recognition of the function blocking anti-alpha   antibody 3H5.	bind
55537	5	7698	6	10	NULL	0	NULL				is substituted for			Asp					alanine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_43_25866_s_149	7592772	3) Alanine substitution of Asp ,  Tyr , or deletion of residues  Phe -Tyr   (delta246-252)  abolished the binding of alpha beta   to iC3b as  well as the recognition of the function blocking anti-alpha   antibody 3H5.	bind
55538	6	7698	6	10	NULL	0	NULL				is substituted for			Tyr					alanine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_43_25866_s_149	7592772	3) Alanine substitution of Asp ,  Tyr , or deletion of residues  Phe -Tyr   (delta246-252)  abolished the binding of alpha beta   to iC3b as  well as the recognition of the function blocking anti-alpha   antibody 3H5.	bind
55539	7	7698	6	10	NULL	0	NULL	statement 5			block					anti-alpha antibody 3H5					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_43_25866_s_149	7592772	3) Alanine substitution of Asp ,  Tyr , or deletion of residues  Phe -Tyr   (delta246-252)  abolished the binding of alpha beta   to iC3b as  well as the recognition of the function blocking anti-alpha   antibody 3H5.	bind
55540	8	7698	6	10	NULL	0	NULL	statement 6			block					anti-alpha antibody 3H5					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_43_25866_s_149	7592772	3) Alanine substitution of Asp ,  Tyr , or deletion of residues  Phe -Tyr   (delta246-252)  abolished the binding of alpha beta   to iC3b as  well as the recognition of the function blocking anti-alpha   antibody 3H5.	bind
55541	9	7698	6	10	NULL	0	NULL			deletion of	block			\tresidues Phe -Tyr (delta246-252)		anti-alpha antibody 3H5					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_43_25866_s_149	7592772	3) Alanine substitution of Asp ,  Tyr , or deletion of residues  Phe -Tyr   (delta246-252)  abolished the binding of alpha beta   to iC3b as  well as the recognition of the function blocking anti-alpha   antibody 3H5.	bind
30983	1	7699	5	13	NULL	NULL	NULL	ANP	GP		inhibit					NF-kappaB	GP	binding activity of			NULL	LPS-activated murine macrophages	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_22_13444_s_226	9593677	3) ANP inhibited binding activity of NF-kappaB, the predominant transcription factor for iNOS induction in LPS-activated murine macrophages ( 36).	bind
30988	2	7699	5	13	NULL	NULL	NULL	NF-kappaB	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_22_13444_s_226	9593677	3) ANP inhibited binding activity of NF-kappaB, the predominant transcription factor for iNOS induction in LPS-activated murine macrophages ( 36).	bind
30989	3	7699	5	13	NULL	NULL	NULL	NF-kappaB	GP		induces					iNOS	GP				NULL	in LPS-activated murine macrophages	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_22_13444_s_226	9593677	3) ANP inhibited binding activity of NF-kappaB, the predominant transcription factor for iNOS induction in LPS-activated murine macrophages ( 36).	bind
23931	1	7699	6	10	NULL	0	NULL	ANP			inhibits					NF-kappaB		binding activity of 			NULL	LPS-activated murine macrophages	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_22_13444_s_226	9593677	3) ANP inhibited binding activity of NF-kappaB, the predominant transcription factor for iNOS induction in LPS-activated murine macrophages ( 36).	bind
23932	2	7699	6	NULL	NULL	0	NULL	NF-kappaB	NULL		induces	NULL				iNOS 	NULL				NULL	LPS-activated murine macrophages	0	NULL	NULL	NULL	gw60_jbiolchem_273_22_13444_s_226	9593677	3) ANP inhibited binding activity of NF-kappaB, the predominant transcription factor for iNOS induction in LPS-activated murine macrophages ( 36).	bind
46740	3	7699	6	10	NULL	0	NULL	NF-kappaB	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_22_13444_s_226	9593677	3) ANP inhibited binding activity of NF-kappaB, the predominant transcription factor for iNOS induction in LPS-activated murine macrophages ( 36).	bind
30991	1	7700	5	13	NULL	NULL	NULL	Skp	GP		bind					OmpA	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_11_9092_s_40	12509434	3) At which stoichiometries and how strong does Skp (or LPS) bind to OmpA?	bind
30992	2	7700	5	13	NULL	NULL	NULL	LPS	Chemical		bind					OmpA	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_11_9092_s_40	12509434	3) At which stoichiometries and how strong does Skp (or LPS) bind to OmpA?	bind
30994	3	7700	5	13	NULL	NULL	NULL	statement 1	Process		is alternative to 					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_11_9092_s_40	12509434	3) At which stoichiometries and how strong does Skp (or LPS) bind to OmpA?	bind
23933	1	7700	6	NULL	NULL	0	NULL	Skp	NULL		bind	NULL				OmpA	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_11_9092_s_40	12509434	3) At which stoichiometries and how strong does Skp (or LPS) bind to OmpA?	bind
23934	2	7700	6	NULL	NULL	0	NULL	LPS	NULL		bind	NULL				OmpA	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_11_9092_s_40	12509434	3) At which stoichiometries and how strong does Skp (or LPS) bind to OmpA?	bind
46741	3	7700	6	10	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_11_9092_s_40	12509434	3) At which stoichiometries and how strong does Skp (or LPS) bind to OmpA?	bind
30996	1	7701	5	13	NULL	NULL	NULL	UTI	Chemical		bind					UTI-BP40	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_17_13650_s_247	11278581	3) Because UTI can bind UTI-BP40 ( K d = ~250 nM) and UTI-BP45 ( K d = ~10 nM), we believe that UTI binds initially to UTI-BP45 and subsequently to UTI-BP40, and 4) although essential for binding, either the amino terminus alone or the C4S side chain alone is not sufficient for UTI-dependent suppression of PMA-activated up-regulation of uPA.	bind
30998	2	7701	5	13	NULL	NULL	NULL	UTI	Chemical		bind					UTI-BP45	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_17_13650_s_247	11278581	3) Because UTI can bind UTI-BP40 ( K d = ~250 nM) and UTI-BP45 ( K d = ~10 nM), we believe that UTI binds initially to UTI-BP45 and subsequently to UTI-BP40, and 4) although essential for binding, either the amino terminus alone or the C4S side chain alone is not sufficient for UTI-dependent suppression of PMA-activated up-regulation of uPA.	bind
30999	3	7701	5	13	NULL	NULL	NULL	statement 2	Process		is followed by					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_17_13650_s_247	11278581	3) Because UTI can bind UTI-BP40 ( K d = ~250 nM) and UTI-BP45 ( K d = ~10 nM), we believe that UTI binds initially to UTI-BP45 and subsequently to UTI-BP40, and 4) although essential for binding, either the amino terminus alone or the C4S side chain alone is not sufficient for UTI-dependent suppression of PMA-activated up-regulation of uPA.	bind
31001	4	7701	5	13	NULL	NULL	NULL	PMA	Chemical		activate					uPA	GP	up-regulation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_17_13650_s_247	11278581	3) Because UTI can bind UTI-BP40 ( K d = ~250 nM) and UTI-BP45 ( K d = ~10 nM), we believe that UTI binds initially to UTI-BP45 and subsequently to UTI-BP40, and 4) although essential for binding, either the amino terminus alone or the C4S side chain alone is not sufficient for UTI-dependent suppression of PMA-activated up-regulation of uPA.	bind
31002	5	7701	5	13	NULL	NULL	NULL	statement 4	Process	suppression of	is dependent on					UTI	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_17_13650_s_247	11278581	3) Because UTI can bind UTI-BP40 ( K d = ~250 nM) and UTI-BP45 ( K d = ~10 nM), we believe that UTI binds initially to UTI-BP45 and subsequently to UTI-BP40, and 4) although essential for binding, either the amino terminus alone or the C4S side chain alone is not sufficient for UTI-dependent suppression of PMA-activated up-regulation of uPA.	bind
31005	6	7701	5	13	NULL	NULL	NULL				is not sufficient for			amino terminus		statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_17_13650_s_247	11278581	3) Because UTI can bind UTI-BP40 ( K d = ~250 nM) and UTI-BP45 ( K d = ~10 nM), we believe that UTI binds initially to UTI-BP45 and subsequently to UTI-BP40, and 4) although essential for binding, either the amino terminus alone or the C4S side chain alone is not sufficient for UTI-dependent suppression of PMA-activated up-regulation of uPA.	bind
31007	7	7701	5	13	NULL	NULL	NULL				is not sufficient for			C4S side chain		statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_17_13650_s_247	11278581	3) Because UTI can bind UTI-BP40 ( K d = ~250 nM) and UTI-BP45 ( K d = ~10 nM), we believe that UTI binds initially to UTI-BP45 and subsequently to UTI-BP40, and 4) although essential for binding, either the amino terminus alone or the C4S side chain alone is not sufficient for UTI-dependent suppression of PMA-activated up-regulation of uPA.	bind
24021	1	7701	6	NULL	NULL	0	NULL	UTI	NULL		bind	NULL				UTI-BP40	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_17_13650_s_247	11278581	3) Because UTI can bind UTI-BP40 ( K d = ~250 nM) and UTI-BP45 ( K d = ~10 nM), we believe that UTI binds initially to UTI-BP45 and subsequently to UTI-BP40, and 4) although essential for binding, either the amino terminus alone or the C4S side chain alone is not sufficient for UTI-dependent suppression of PMA-activated up-regulation of uPA.	bind
24022	2	7701	6	NULL	NULL	0	NULL	UTI	NULL		bind	NULL				UTI-BP45	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_17_13650_s_247	11278581	3) Because UTI can bind UTI-BP40 ( K d = ~250 nM) and UTI-BP45 ( K d = ~10 nM), we believe that UTI binds initially to UTI-BP45 and subsequently to UTI-BP40, and 4) although essential for binding, either the amino terminus alone or the C4S side chain alone is not sufficient for UTI-dependent suppression of PMA-activated up-regulation of uPA.	bind
24023	3	7701	6	NULL	NULL	0	NULL	statement 2	NULL		occurs before	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_17_13650_s_247	11278581	3) Because UTI can bind UTI-BP40 ( K d = ~250 nM) and UTI-BP45 ( K d = ~10 nM), we believe that UTI binds initially to UTI-BP45 and subsequently to UTI-BP40, and 4) although essential for binding, either the amino terminus alone or the C4S side chain alone is not sufficient for UTI-dependent suppression of PMA-activated up-regulation of uPA.	bind
24024	4	7701	6	NULL	NULL	0	NULL	PMA	NULL		activates	NULL				uPA	NULL	up-regulation of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_17_13650_s_247	11278581	3) Because UTI can bind UTI-BP40 ( K d = ~250 nM) and UTI-BP45 ( K d = ~10 nM), we believe that UTI binds initially to UTI-BP45 and subsequently to UTI-BP40, and 4) although essential for binding, either the amino terminus alone or the C4S side chain alone is not sufficient for UTI-dependent suppression of PMA-activated up-regulation of uPA.	bind
24025	5	7701	6	NULL	NULL	0	NULL	statement 4	NULL		is suppressed by	NULL				UTI	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_17_13650_s_247	11278581	3) Because UTI can bind UTI-BP40 ( K d = ~250 nM) and UTI-BP45 ( K d = ~10 nM), we believe that UTI binds initially to UTI-BP45 and subsequently to UTI-BP40, and 4) although essential for binding, either the amino terminus alone or the C4S side chain alone is not sufficient for UTI-dependent suppression of PMA-activated up-regulation of uPA.	bind
24026	6	7701	6	NULL	NULL	0	NULL		NULL		is not sufficient for	NULL		amino terminus		statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_17_13650_s_247	11278581	3) Because UTI can bind UTI-BP40 ( K d = ~250 nM) and UTI-BP45 ( K d = ~10 nM), we believe that UTI binds initially to UTI-BP45 and subsequently to UTI-BP40, and 4) although essential for binding, either the amino terminus alone or the C4S side chain alone is not sufficient for UTI-dependent suppression of PMA-activated up-regulation of uPA.	bind
24027	7	7701	6	NULL	NULL	0	NULL		NULL	alone	is not sufficient for	NULL		C4S side chain		statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_17_13650_s_247	11278581	3) Because UTI can bind UTI-BP40 ( K d = ~250 nM) and UTI-BP45 ( K d = ~10 nM), we believe that UTI binds initially to UTI-BP45 and subsequently to UTI-BP40, and 4) although essential for binding, either the amino terminus alone or the C4S side chain alone is not sufficient for UTI-dependent suppression of PMA-activated up-regulation of uPA.	bind
31008	1	7702	5	13	NULL	NULL	NULL	hsp70	GP	purified	bind					K8/18	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_915_s_207	7529764	3) Binding of purified hsp70 to K8/18 is  partially facilitated by ATP, and release of the hsp/c70-K8/18 complex  in detergent cell lysates or in isolated immunoprecipitates requires  Mg-ATP and ATP hydrolysis.	bind
31009	2	7702	5	13	NULL	NULL	NULL	ATP	Chemical		facilitate		partially			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_915_s_207	7529764	3) Binding of purified hsp70 to K8/18 is  partially facilitated by ATP, and release of the hsp/c70-K8/18 complex  in detergent cell lysates or in isolated immunoprecipitates requires  Mg-ATP and ATP hydrolysis.	bind
31010	3	7702	5	13	NULL	NULL	NULL	hsp/c70-K8/18 complex	GP	release of	requires					Mg-ATP	Chemical				NULL	in detergent cell lysates	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_915_s_207	7529764	3) Binding of purified hsp70 to K8/18 is  partially facilitated by ATP, and release of the hsp/c70-K8/18 complex  in detergent cell lysates or in isolated immunoprecipitates requires  Mg-ATP and ATP hydrolysis.	bind
31011	4	7702	5	13	NULL	NULL	NULL	hsp/c70-K8/18 complex	GP	release of	requires					ATP 	Chemical	hydrolysis of			NULL	in detergent cell lysates	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_915_s_207	7529764	3) Binding of purified hsp70 to K8/18 is  partially facilitated by ATP, and release of the hsp/c70-K8/18 complex  in detergent cell lysates or in isolated immunoprecipitates requires  Mg-ATP and ATP hydrolysis.	bind
31013	5	7702	5	13	NULL	NULL	NULL	hsp/c70-K8/18 complex	GP	release of	requires					Mg-ATP	Chemical				NULL	in isolated immunoprecipitates 	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_915_s_207	7529764	3) Binding of purified hsp70 to K8/18 is  partially facilitated by ATP, and release of the hsp/c70-K8/18 complex  in detergent cell lysates or in isolated immunoprecipitates requires  Mg-ATP and ATP hydrolysis.	bind
31015	6	7702	5	13	NULL	NULL	NULL	hsp/c70-K8/18 complex	GP	release of	requires					ATP	Chemical	hydrolysis of			NULL	in isolated immunoprecipitates 	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_915_s_207	7529764	3) Binding of purified hsp70 to K8/18 is  partially facilitated by ATP, and release of the hsp/c70-K8/18 complex  in detergent cell lysates or in isolated immunoprecipitates requires  Mg-ATP and ATP hydrolysis.	bind
24028	1	7702	6	NULL	NULL	0	NULL	hsp70	NULL	purified	bind	NULL				K8/18	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_2_915_s_207	7529764	3) Binding of purified hsp70 to K8/18 is  partially facilitated by ATP, and release of the hsp/c70-K8/18 complex  in detergent cell lysates or in isolated immunoprecipitates requires  Mg-ATP and ATP hydrolysis.	bind
24029	2	7702	6	NULL	NULL	0	NULL	statement 1	NULL		is facilitated by	NULL	partially			ATP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_2_915_s_207	7529764	3) Binding of purified hsp70 to K8/18 is  partially facilitated by ATP, and release of the hsp/c70-K8/18 complex  in detergent cell lysates or in isolated immunoprecipitates requires  Mg-ATP and ATP hydrolysis.	bind
24030	3	7702	6	10	NULL	0	NULL	hsp/c70-K8/18 complex	NULL	release of	requires	NULL				Mg-ATP	NULL	hydrolysis of			NULL	detergent cell lysates	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_915_s_207	7529764	3) Binding of purified hsp70 to K8/18 is  partially facilitated by ATP, and release of the hsp/c70-K8/18 complex  in detergent cell lysates or in isolated immunoprecipitates requires  Mg-ATP and ATP hydrolysis.	bind
24031	4	7702	6	10	NULL	0	NULL	hsp/c70-K8/18 complex	NULL	release of	requires	NULL				ATP	NULL	hydrolysis of			NULL	detergent cell lysates	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_915_s_207	7529764	3) Binding of purified hsp70 to K8/18 is  partially facilitated by ATP, and release of the hsp/c70-K8/18 complex  in detergent cell lysates or in isolated immunoprecipitates requires  Mg-ATP and ATP hydrolysis.	bind
46742	5	7702	6	10	NULL	0	NULL	hsp/c70-K8/18 complex	NULL	release of	requires	NULL				Mg-ATP	NULL	hydrolysis of			NULL	in isolated immunoprecipitates	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_915_s_207	7529764	3) Binding of purified hsp70 to K8/18 is  partially facilitated by ATP, and release of the hsp/c70-K8/18 complex  in detergent cell lysates or in isolated immunoprecipitates requires  Mg-ATP and ATP hydrolysis.	bind
46743	6	7702	6	10	NULL	0	NULL	hsp/c70-K8/18 complex 		release of	requires					ATP		hydrolysis of			NULL	in isolated immunoprecipitates	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_915_s_207	7529764	3) Binding of purified hsp70 to K8/18 is  partially facilitated by ATP, and release of the hsp/c70-K8/18 complex  in detergent cell lysates or in isolated immunoprecipitates requires  Mg-ATP and ATP hydrolysis.	bind
24032	1	7703	6	NULL	NULL	0	NULL	Stat3	NULL		bind	NULL		SH2 domain		pY XXQ-containing peptide	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_18967_s_28	14966128	3) Binding of Stat3 SH2 to pY XXQ-containing peptides does not require the side chains of Glu-638, Tyr-640, and Tyr-657 or Tyr-657, Cys-687, Ser-691, and Glu-692 proposed to form pocket 2 in the Chakraborty  et al. ( ) and Hemmann  et al. ( ) models, respectively.	bind
24033	2	7703	6	10	NULL	0	NULL	statement 1	NULL		does not require	NULL					NULL	side chains of	 Glu-638		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_18967_s_28	14966128	3) Binding of Stat3 SH2 to pY XXQ-containing peptides does not require the side chains of Glu-638, Tyr-640, and Tyr-657 or Tyr-657, Cys-687, Ser-691, and Glu-692 proposed to form pocket 2 in the Chakraborty  et al. ( ) and Hemmann  et al. ( ) models, respectively.	bind
24034	3	7703	6	10	NULL	0	NULL	statement 1	NULL		does not require	NULL					NULL	side chains of 	Tyr-640		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_18967_s_28	14966128	3) Binding of Stat3 SH2 to pY XXQ-containing peptides does not require the side chains of Glu-638, Tyr-640, and Tyr-657 or Tyr-657, Cys-687, Ser-691, and Glu-692 proposed to form pocket 2 in the Chakraborty  et al. ( ) and Hemmann  et al. ( ) models, respectively.	bind
46748	4	7703	6	10	NULL	0	NULL	statement 1	NULL		does not require	NULL					NULL	side chains of	Tyr-657		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_18_18967_s_28	14966128	3) Binding of Stat3 SH2 to pY XXQ-containing peptides does not require the side chains of Glu-638, Tyr-640, and Tyr-657 or Tyr-657, Cys-687, Ser-691, and Glu-692 proposed to form pocket 2 in the Chakraborty  et al. ( ) and Hemmann  et al. ( ) models, respectively.	bind
46749	5	7703	6	10	NULL	0	NULL	statement 1	NULL		does not require	NULL					NULL	side chains of	Cys-687		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_18_18967_s_28	14966128	3) Binding of Stat3 SH2 to pY XXQ-containing peptides does not require the side chains of Glu-638, Tyr-640, and Tyr-657 or Tyr-657, Cys-687, Ser-691, and Glu-692 proposed to form pocket 2 in the Chakraborty  et al. ( ) and Hemmann  et al. ( ) models, respectively.	bind
46750	6	7703	6	10	NULL	0	NULL	statement 1	NULL		does not require	NULL					NULL	side chains of	Ser-691		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_18_18967_s_28	14966128	3) Binding of Stat3 SH2 to pY XXQ-containing peptides does not require the side chains of Glu-638, Tyr-640, and Tyr-657 or Tyr-657, Cys-687, Ser-691, and Glu-692 proposed to form pocket 2 in the Chakraborty  et al. ( ) and Hemmann  et al. ( ) models, respectively.	bind
46751	7	7703	6	10	NULL	0	NULL	statement 1	NULL		does not require	NULL					NULL	side chains of	Glu-692		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_18_18967_s_28	14966128	3) Binding of Stat3 SH2 to pY XXQ-containing peptides does not require the side chains of Glu-638, Tyr-640, and Tyr-657 or Tyr-657, Cys-687, Ser-691, and Glu-692 proposed to form pocket 2 in the Chakraborty  et al. ( ) and Hemmann  et al. ( ) models, respectively.	bind
31071	1	7704	5	13	NULL	NULL	NULL	p53	GP		bind					PKD1 gene	GP	endogenous		p53 consensus-like DNA sequences	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_42_31234_s_276	16931520	3) ChIP assays performed in p53-transfected cells reveals that p53 binds the endogenous  PKD1 gene in regions containing p53 consensus-like DNA sequences.	bind
24036	1	7704	6	10	NULL	0	NULL	p53	NULL		bind	NULL				PKD1 gene	NULL	endogenous		p53 consensus-like DNA sequences	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_42_31234_s_276	16931520	3) ChIP assays performed in p53-transfected cells reveals that p53 binds the endogenous  PKD1 gene in regions containing p53 consensus-like DNA sequences.	bind
31073	1	7705	5	13	NULL	NULL	NULL	lin-benzo-ADP	Chemical		bind					F1	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_267_3_1530942_s_6	1530942	3) Fluorescence  properties of lin-benzo-ADP bound to F1 differed widely, depending on  the residue present at position beta 331.	bind
24037	1	7705	6	NULL	NULL	0	NULL	lin-benzo-ADP	NULL		bind	NULL				F1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_267_3_1530942_s_6	1530942	3) Fluorescence  properties of lin-benzo-ADP bound to F1 differed widely, depending on  the residue present at position beta 331.	bind
31075	1	7706	5	13	NULL	NULL	NULL	GR	GP		bind							putative;;mitochondrial		GR elements	NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_steroids_61_4_8733006_s_9	8733006	3) Gel  shift analysis has demonstrated binding of GR to putative mitochondrial  GR elements.	bind
24038	1	7706	6	10	NULL	0	NULL	GR	NULL		bind	NULL					NULL	putative;;mitochondrial		GR elements	NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_steroids_61_4_8733006_s_9	8733006	3) Gel  shift analysis has demonstrated binding of GR to putative mitochondrial  GR elements.	bind
31076	1	7707	5	13	NULL	NULL	NULL	DAG	Chemical		bind		predominantly						C1a domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_26_17815_s_480	16613842	3) In concert, DAG binding with C1 domains (predominantly C1a), Thr588 phosphorylation, and the protein configuration within the PH domain create a conformation that allows expression of maximal kinase activity.	bind
24039	1	7707	6	NULL	NULL	0	NULL	DAG	NULL		bind	NULL					NULL		C1 domain		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_26_17815_s_480	16613842	3) In concert, DAG binding with C1 domains (predominantly C1a), Thr588 phosphorylation, and the protein configuration within the PH domain create a conformation that allows expression of maximal kinase activity.	bind
31079	1	7708	5	13	NULL	NULL	NULL	SOCS3	GP		does not bind					OSMR	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_13_8458_s_237	16459330	3) in contrast to the inhibitory mechanisms of SOCS3 described so far, no binding of SOCS3 to the OSMR was found, but a direct association with JAK1 was found.	bind
31082	2	7708	5	13	NULL	NULL	NULL	SOCS3	GP		associates with		directly			JAK1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_13_8458_s_237	16459330	3) in contrast to the inhibitory mechanisms of SOCS3 described so far, no binding of SOCS3 to the OSMR was found, but a direct association with JAK1 was found.	bind
24043	1	7708	6	NULL	NULL	0	NULL	SOCS3	NULL		does not bind	NULL				OSMR	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_13_8458_s_237	16459330	3) in contrast to the inhibitory mechanisms of SOCS3 described so far, no binding of SOCS3 to the OSMR was found, but a direct association with JAK1 was found.	bind
24044	2	7708	6	NULL	NULL	0	NULL	SOCS3	NULL		associates with	NULL	directly			JAK1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_13_8458_s_237	16459330	3) in contrast to the inhibitory mechanisms of SOCS3 described so far, no binding of SOCS3 to the OSMR was found, but a direct association with JAK1 was found.	bind
31083	1	7709	5	13	NULL	NULL	NULL	LPS	Chemical		bind					CD14	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_17_9904_s_7	7537270	3) In contrast, substoichiometric concentrations of dLPS (1  ng/ml) inhibited LPS-induced (3 ng/ml) interleukin-8 release without  blocking LPS binding to CD14.	bind
31084	2	7709	5	13	NULL	NULL	NULL	LPS	Chemical		induces					interleukin-8	GP	release of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_17_9904_s_7	7537270	3) In contrast, substoichiometric concentrations of dLPS (1  ng/ml) inhibited LPS-induced (3 ng/ml) interleukin-8 release without  blocking LPS binding to CD14.	bind
31085	3	7709	5	13	NULL	NULL	NULL	dLPS	Chemical		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_17_9904_s_7	7537270	3) In contrast, substoichiometric concentrations of dLPS (1  ng/ml) inhibited LPS-induced (3 ng/ml) interleukin-8 release without  blocking LPS binding to CD14.	bind
31086	4	7709	5	13	NULL	NULL	NULL	statement 3	Process		occurs without					statement 1	Process	blocking			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_17_9904_s_7	7537270	3) In contrast, substoichiometric concentrations of dLPS (1  ng/ml) inhibited LPS-induced (3 ng/ml) interleukin-8 release without  blocking LPS binding to CD14.	bind
24045	1	7709	6	NULL	NULL	0	NULL	LPS	NULL		bind	NULL				CD14	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_17_9904_s_7	7537270	3) In contrast, substoichiometric concentrations of dLPS (1  ng/ml) inhibited LPS-induced (3 ng/ml) interleukin-8 release without  blocking LPS binding to CD14.	bind
24046	2	7709	6	NULL	NULL	0	NULL	LPS	NULL		induces	NULL				interleukin-8	NULL	release of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_17_9904_s_7	7537270	3) In contrast, substoichiometric concentrations of dLPS (1  ng/ml) inhibited LPS-induced (3 ng/ml) interleukin-8 release without  blocking LPS binding to CD14.	bind
24047	3	7709	6	NULL	NULL	0	NULL	dLPS	NULL		inhibits	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_17_9904_s_7	7537270	3) In contrast, substoichiometric concentrations of dLPS (1  ng/ml) inhibited LPS-induced (3 ng/ml) interleukin-8 release without  blocking LPS binding to CD14.	bind
24048	4	7709	6	10	NULL	0	NULL	statement 3	NULL		occurs without 	NULL				statement 1	NULL	blocking			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_17_9904_s_7	7537270	3) In contrast, substoichiometric concentrations of dLPS (1  ng/ml) inhibited LPS-induced (3 ng/ml) interleukin-8 release without  blocking LPS binding to CD14.	bind
31087	1	7710	5	13	NULL	NULL	NULL	eptifibatide	Chemical		induce					GPIIb/IIa	GP	conformational change of			NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_308_3_1002_s_187	14617694	3) In the presence of fibrinogen, the eptifibatide-induced conformational change of GPIIb/IIa is only partially reversible upon dissociation of the GPIIb/IIa blocker, as detected by the binding of a mAb specific for a LIBS, the binding of the ligand-mimetic mAb Pac-1, and the binding of the GPIIb/IIIa ligand fibrinogen.	bind
31088	2	7710	5	13	NULL	NULL	NULL	statement 1	Process		in the presence of					fibrinogen	GP				NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_308_3_1002_s_187	14617694	3) In the presence of fibrinogen, the eptifibatide-induced conformational change of GPIIb/IIa is only partially reversible upon dissociation of the GPIIb/IIa blocker, as detected by the binding of a mAb specific for a LIBS, the binding of the ligand-mimetic mAb Pac-1, and the binding of the GPIIb/IIIa ligand fibrinogen.	bind
31089	3	7710	5	13	NULL	NULL	NULL	GPIIb/IIa blocker	Chemical	dissociation of	reverse		partially			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_308_3_1002_s_187	14617694	3) In the presence of fibrinogen, the eptifibatide-induced conformational change of GPIIb/IIa is only partially reversible upon dissociation of the GPIIb/IIa blocker, as detected by the binding of a mAb specific for a LIBS, the binding of the ligand-mimetic mAb Pac-1, and the binding of the GPIIb/IIIa ligand fibrinogen.	bind
24049	1	7710	6	NULL	NULL	0	NULL	eptifibatide	NULL		induces	NULL				GPIIb/IIa	NULL	conformational change of			NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_308_3_1002_s_187	14617694	3) In the presence of fibrinogen, the eptifibatide-induced conformational change of GPIIb/IIa is only partially reversible upon dissociation of the GPIIb/IIa blocker, as detected by the binding of a mAb specific for a LIBS, the binding of the ligand-mimetic mAb Pac-1, and the binding of the GPIIb/IIIa ligand fibrinogen.	bind
24050	2	7710	6	10	NULL	0	NULL	GPIIb/IIa blocker	NULL	dissociation of	reverse	NULL	partially			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_308_3_1002_s_187	14617694	3) In the presence of fibrinogen, the eptifibatide-induced conformational change of GPIIb/IIa is only partially reversible upon dissociation of the GPIIb/IIa blocker, as detected by the binding of a mAb specific for a LIBS, the binding of the ligand-mimetic mAb Pac-1, and the binding of the GPIIb/IIIa ligand fibrinogen.	bind
24051	3	7710	6	10	NULL	0	NULL	statement 1	NULL		in the presence of	NULL				fibrinogen	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_308_3_1002_s_187	14617694	3) In the presence of fibrinogen, the eptifibatide-induced conformational change of GPIIb/IIa is only partially reversible upon dissociation of the GPIIb/IIa blocker, as detected by the binding of a mAb specific for a LIBS, the binding of the ligand-mimetic mAb Pac-1, and the binding of the GPIIb/IIIa ligand fibrinogen.	bind
31090	1	7711	5	13	NULL	NULL	NULL	Src's	GP		interacts with			SH2 domain		tyrosine	AminoAcid	phosphorylated			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_22_16788_s_223	10747984	3) Interaction of Src's SH2 domain with a phosphorylated tyrosine on another protein could outcompete the binding of the SH2 domain to the COOH-terminal tyrosine, and thus disrupt the closed conformation.	bind
31093	2	7711	5	13	NULL	NULL	NULL				bind			SH2 domain		tyrosine	AminoAcid		COOH-terminus		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_22_16788_s_223	10747984	3) Interaction of Src's SH2 domain with a phosphorylated tyrosine on another protein could outcompete the binding of the SH2 domain to the COOH-terminal tyrosine, and thus disrupt the closed conformation.	bind
31094	3	7711	5	13	NULL	NULL	NULL	statement 1	Process		outcompetes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_22_16788_s_223	10747984	3) Interaction of Src's SH2 domain with a phosphorylated tyrosine on another protein could outcompete the binding of the SH2 domain to the COOH-terminal tyrosine, and thus disrupt the closed conformation.	bind
31095	4	7711	5	13	NULL	NULL	NULL	statement 3	Process		disrupt					conformation	Process	closed			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_22_16788_s_223	10747984	3) Interaction of Src's SH2 domain with a phosphorylated tyrosine on another protein could outcompete the binding of the SH2 domain to the COOH-terminal tyrosine, and thus disrupt the closed conformation.	bind
24052	1	7711	6	NULL	NULL	0	NULL	Src	NULL		interacts with	NULL		SH2 domain		tyrosine	NULL	phosphorylated			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_22_16788_s_223	10747984	3) Interaction of Src's SH2 domain with a phosphorylated tyrosine on another protein could outcompete the binding of the SH2 domain to the COOH-terminal tyrosine, and thus disrupt the closed conformation.	bind
24053	2	7711	6	NULL	NULL	0	NULL		NULL		bind	NULL		SH2 domain			NULL		COOH terminal tyrosine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_22_16788_s_223	10747984	3) Interaction of Src's SH2 domain with a phosphorylated tyrosine on another protein could outcompete the binding of the SH2 domain to the COOH-terminal tyrosine, and thus disrupt the closed conformation.	bind
24054	3	7711	6	NULL	NULL	0	NULL	statement 1	NULL		out competes	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_22_16788_s_223	10747984	3) Interaction of Src's SH2 domain with a phosphorylated tyrosine on another protein could outcompete the binding of the SH2 domain to the COOH-terminal tyrosine, and thus disrupt the closed conformation.	bind
31096	1	7712	5	13	NULL	NULL	NULL	prothrombin	GP		bind					FXI	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_31954_s_226	10924522	3) PF1.2 inhibits the binding of prothrombin to FXI (with a IC50 of 5 x 10-7M), whereas PF1 has no effect (Fig.  1 B, Table  I).	bind
31097	2	7712	5	13	NULL	NULL	NULL	PF1.2	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_31954_s_226	10924522	3) PF1.2 inhibits the binding of prothrombin to FXI (with a IC50 of 5 x 10-7M), whereas PF1 has no effect (Fig.  1 B, Table  I).	bind
31098	3	7712	5	13	NULL	NULL	NULL	PF1	GP		does not effect					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_31954_s_226	10924522	3) PF1.2 inhibits the binding of prothrombin to FXI (with a IC50 of 5 x 10-7M), whereas PF1 has no effect (Fig.  1 B, Table  I).	bind
24055	1	7712	6	NULL	NULL	0	NULL	prothrombin	NULL		bind	NULL				FXI	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_41_31954_s_226	10924522	3) PF1.2 inhibits the binding of prothrombin to FXI (with a IC50 of 5 x 10-7M), whereas PF1 has no effect (Fig.  1 B, Table  I).	bind
24056	2	7712	6	NULL	NULL	0	NULL	PF1.2	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_41_31954_s_226	10924522	3) PF1.2 inhibits the binding of prothrombin to FXI (with a IC50 of 5 x 10-7M), whereas PF1 has no effect (Fig.  1 B, Table  I).	bind
24057	3	7712	6	NULL	NULL	0	NULL	PF1	NULL		has no effect on	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_41_31954_s_226	10924522	3) PF1.2 inhibits the binding of prothrombin to FXI (with a IC50 of 5 x 10-7M), whereas PF1 has no effect (Fig.  1 B, Table  I).	bind
31099	1	7713	5	13	NULL	NULL	NULL	alphaMbeta2	GP	wild-type	bind					C3bi	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_36_34395_s_8	12816955	3) Polyclonal antibodies recognizing sequences  within the W4 blade significantly blocked C3bi binding by wild-type  alphaMbeta2.	bind
31100	2	7713	5	13	NULL	NULL	NULL	polyclonal antibodies	GP		recognize								sequences within W4 blade		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_36_34395_s_8	12816955	3) Polyclonal antibodies recognizing sequences  within the W4 blade significantly blocked C3bi binding by wild-type  alphaMbeta2.	bind
46752	3	7713	5	13	NULL	NULL	NULL	statement 2	Process		blocks		significantly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_36_34395_s_8	12816955	3) Polyclonal antibodies recognizing sequences  within the W4 blade significantly blocked C3bi binding by wild-type  alphaMbeta2.	bind
24059	1	7713	6	NULL	NULL	0	NULL	C3bi	NULL		bind	NULL				alphaMbeta2	NULL	wild type			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_36_34395_s_8	12816955	3) Polyclonal antibodies recognizing sequences  within the W4 blade significantly blocked C3bi binding by wild-type  alphaMbeta2.	bind
24060	2	7713	6	NULL	NULL	0	NULL	Polyclonal antibodies	NULL		recognize	NULL					NULL		sequences within W4 blade		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_36_34395_s_8	12816955	3) Polyclonal antibodies recognizing sequences  within the W4 blade significantly blocked C3bi binding by wild-type  alphaMbeta2.	bind
24061	3	7713	6	NULL	NULL	0	NULL	statement 2	NULL		blocks	NULL	significantly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_36_34395_s_8	12816955	3) Polyclonal antibodies recognizing sequences  within the W4 blade significantly blocked C3bi binding by wild-type  alphaMbeta2.	bind
31101	1	7714	5	13	NULL	NULL	NULL	PP2A	GP		bind					tau	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_250	10464280	3) PP2A binds to tau and MTs through distinct sites and therefore might be able to anchor tau to MTs. 4) Since MTs and PP2A compete for binding to the same region on tau and binding of PP2A to MTs inhibits its catalytic activity, PP2A can efficiently dephosphorylate tau only when neither protein is bound to MTs. Depolymerization of MTs or dissociation of PP2A from MTs thus potentiates the phosphatase activity of PP2A for soluble tau.	bind
31102	2	7714	5	13	NULL	NULL	NULL	PP2A	GP		bind					MTs	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_250	10464280	3) PP2A binds to tau and MTs through distinct sites and therefore might be able to anchor tau to MTs. 4) Since MTs and PP2A compete for binding to the same region on tau and binding of PP2A to MTs inhibits its catalytic activity, PP2A can efficiently dephosphorylate tau only when neither protein is bound to MTs. Depolymerization of MTs or dissociation of PP2A from MTs thus potentiates the phosphatase activity of PP2A for soluble tau.	bind
31103	3	7714	5	13	NULL	NULL	NULL	statement 1 	Process		occurs through					distinct sites	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_250	10464280	3) PP2A binds to tau and MTs through distinct sites and therefore might be able to anchor tau to MTs. 4) Since MTs and PP2A compete for binding to the same region on tau and binding of PP2A to MTs inhibits its catalytic activity, PP2A can efficiently dephosphorylate tau only when neither protein is bound to MTs. Depolymerization of MTs or dissociation of PP2A from MTs thus potentiates the phosphatase activity of PP2A for soluble tau.	bind
31104	4	7714	5	13	NULL	NULL	NULL	tau	GP		is anchored to					MTs	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_250	10464280	3) PP2A binds to tau and MTs through distinct sites and therefore might be able to anchor tau to MTs. 4) Since MTs and PP2A compete for binding to the same region on tau and binding of PP2A to MTs inhibits its catalytic activity, PP2A can efficiently dephosphorylate tau only when neither protein is bound to MTs. Depolymerization of MTs or dissociation of PP2A from MTs thus potentiates the phosphatase activity of PP2A for soluble tau.	bind
31105	5	7714	5	13	NULL	NULL	NULL	PP2A	GP		is required for					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_250	10464280	3) PP2A binds to tau and MTs through distinct sites and therefore might be able to anchor tau to MTs. 4) Since MTs and PP2A compete for binding to the same region on tau and binding of PP2A to MTs inhibits its catalytic activity, PP2A can efficiently dephosphorylate tau only when neither protein is bound to MTs. Depolymerization of MTs or dissociation of PP2A from MTs thus potentiates the phosphatase activity of PP2A for soluble tau.	bind
31106	6	7714	5	13	NULL	NULL	NULL	MTs	CellComponent		bind					tau	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_250	10464280	3) PP2A binds to tau and MTs through distinct sites and therefore might be able to anchor tau to MTs. 4) Since MTs and PP2A compete for binding to the same region on tau and binding of PP2A to MTs inhibits its catalytic activity, PP2A can efficiently dephosphorylate tau only when neither protein is bound to MTs. Depolymerization of MTs or dissociation of PP2A from MTs thus potentiates the phosphatase activity of PP2A for soluble tau.	bind
31107	7	7714	5	13	NULL	NULL	NULL	statement 1	Process		competes with					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_250	10464280	3) PP2A binds to tau and MTs through distinct sites and therefore might be able to anchor tau to MTs. 4) Since MTs and PP2A compete for binding to the same region on tau and binding of PP2A to MTs inhibits its catalytic activity, PP2A can efficiently dephosphorylate tau only when neither protein is bound to MTs. Depolymerization of MTs or dissociation of PP2A from MTs thus potentiates the phosphatase activity of PP2A for soluble tau.	bind
31108	8	7714	5	13	NULL	NULL	NULL	statement 2	Process		inhibit					PP2A	GP	catalytic activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_250	10464280	3) PP2A binds to tau and MTs through distinct sites and therefore might be able to anchor tau to MTs. 4) Since MTs and PP2A compete for binding to the same region on tau and binding of PP2A to MTs inhibits its catalytic activity, PP2A can efficiently dephosphorylate tau only when neither protein is bound to MTs. Depolymerization of MTs or dissociation of PP2A from MTs thus potentiates the phosphatase activity of PP2A for soluble tau.	bind
31109	9	7714	5	13	NULL	NULL	NULL	PP2A	GP		dephosphorylate		efficiently			tau	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_250	10464280	3) PP2A binds to tau and MTs through distinct sites and therefore might be able to anchor tau to MTs. 4) Since MTs and PP2A compete for binding to the same region on tau and binding of PP2A to MTs inhibits its catalytic activity, PP2A can efficiently dephosphorylate tau only when neither protein is bound to MTs. Depolymerization of MTs or dissociation of PP2A from MTs thus potentiates the phosphatase activity of PP2A for soluble tau.	bind
31110	10	7714	5	13	NULL	NULL	NULL	statement 9	Process		occur under conditions of					PP2A	GP	unbound			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_250	10464280	3) PP2A binds to tau and MTs through distinct sites and therefore might be able to anchor tau to MTs. 4) Since MTs and PP2A compete for binding to the same region on tau and binding of PP2A to MTs inhibits its catalytic activity, PP2A can efficiently dephosphorylate tau only when neither protein is bound to MTs. Depolymerization of MTs or dissociation of PP2A from MTs thus potentiates the phosphatase activity of PP2A for soluble tau.	bind
31111	11	7714	5	13	NULL	NULL	NULL	statement 9	Process		occur under conditions of					tau	GP	unbound			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_250	10464280	3) PP2A binds to tau and MTs through distinct sites and therefore might be able to anchor tau to MTs. 4) Since MTs and PP2A compete for binding to the same region on tau and binding of PP2A to MTs inhibits its catalytic activity, PP2A can efficiently dephosphorylate tau only when neither protein is bound to MTs. Depolymerization of MTs or dissociation of PP2A from MTs thus potentiates the phosphatase activity of PP2A for soluble tau.	bind
31112	12	7714	5	13	NULL	NULL	NULL	MTs	CellComponent	depolymerization of	potentiates					PP2A	GP	phosphatase activity			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_250	10464280	3) PP2A binds to tau and MTs through distinct sites and therefore might be able to anchor tau to MTs. 4) Since MTs and PP2A compete for binding to the same region on tau and binding of PP2A to MTs inhibits its catalytic activity, PP2A can efficiently dephosphorylate tau only when neither protein is bound to MTs. Depolymerization of MTs or dissociation of PP2A from MTs thus potentiates the phosphatase activity of PP2A for soluble tau.	bind
31113	13	7714	5	13	NULL	NULL	NULL	PP2A	GP		dissociates from					MTs	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_250	10464280	3) PP2A binds to tau and MTs through distinct sites and therefore might be able to anchor tau to MTs. 4) Since MTs and PP2A compete for binding to the same region on tau and binding of PP2A to MTs inhibits its catalytic activity, PP2A can efficiently dephosphorylate tau only when neither protein is bound to MTs. Depolymerization of MTs or dissociation of PP2A from MTs thus potentiates the phosphatase activity of PP2A for soluble tau.	bind
31114	14	7714	5	13	NULL	NULL	NULL	statement 13	Process		potentiates					PP2A	GP	phosphatase activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_250	10464280	3) PP2A binds to tau and MTs through distinct sites and therefore might be able to anchor tau to MTs. 4) Since MTs and PP2A compete for binding to the same region on tau and binding of PP2A to MTs inhibits its catalytic activity, PP2A can efficiently dephosphorylate tau only when neither protein is bound to MTs. Depolymerization of MTs or dissociation of PP2A from MTs thus potentiates the phosphatase activity of PP2A for soluble tau.	bind
46762	15	7714	5	13	NULL	NULL	NULL	statement 2	Process		occur through					distinct sites	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_250	10464280	3) PP2A binds to tau and MTs through distinct sites and therefore might be able to anchor tau to MTs. 4) Since MTs and PP2A compete for binding to the same region on tau and binding of PP2A to MTs inhibits its catalytic activity, PP2A can efficiently dephosphorylate tau only when neither protein is bound to MTs. Depolymerization of MTs or dissociation of PP2A from MTs thus potentiates the phosphatase activity of PP2A for soluble tau.	bind
24062	1	7714	6	NULL	NULL	0	NULL	PP2A	NULL		bind	NULL				tau	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_250	10464280	3) PP2A binds to tau and MTs through distinct sites and therefore might be able to anchor tau to MTs. 4) Since MTs and PP2A compete for binding to the same region on tau and binding of PP2A to MTs inhibits its catalytic activity, PP2A can efficiently dephosphorylate tau only when neither protein is bound to MTs. Depolymerization of MTs or dissociation of PP2A from MTs thus potentiates the phosphatase activity of PP2A for soluble tau.	bind
24063	2	7714	6	NULL	NULL	0	NULL	PP2A	NULL		bind	NULL				MT	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_250	10464280	3) PP2A binds to tau and MTs through distinct sites and therefore might be able to anchor tau to MTs. 4) Since MTs and PP2A compete for binding to the same region on tau and binding of PP2A to MTs inhibits its catalytic activity, PP2A can efficiently dephosphorylate tau only when neither protein is bound to MTs. Depolymerization of MTs or dissociation of PP2A from MTs thus potentiates the phosphatase activity of PP2A for soluble tau.	bind
24066	3	7714	6	NULL	NULL	0	NULL	tau	NULL		anchored to	NULL				MT	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_250	10464280	3) PP2A binds to tau and MTs through distinct sites and therefore might be able to anchor tau to MTs. 4) Since MTs and PP2A compete for binding to the same region on tau and binding of PP2A to MTs inhibits its catalytic activity, PP2A can efficiently dephosphorylate tau only when neither protein is bound to MTs. Depolymerization of MTs or dissociation of PP2A from MTs thus potentiates the phosphatase activity of PP2A for soluble tau.	bind
24067	4	7714	6	NULL	NULL	0	NULL	Tau	NULL		bind	NULL				MT	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_250	10464280	3) PP2A binds to tau and MTs through distinct sites and therefore might be able to anchor tau to MTs. 4) Since MTs and PP2A compete for binding to the same region on tau and binding of PP2A to MTs inhibits its catalytic activity, PP2A can efficiently dephosphorylate tau only when neither protein is bound to MTs. Depolymerization of MTs or dissociation of PP2A from MTs thus potentiates the phosphatase activity of PP2A for soluble tau.	bind
24068	5	7714	6	NULL	NULL	0	NULL	statement 2	NULL		competes	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_250	10464280	3) PP2A binds to tau and MTs through distinct sites and therefore might be able to anchor tau to MTs. 4) Since MTs and PP2A compete for binding to the same region on tau and binding of PP2A to MTs inhibits its catalytic activity, PP2A can efficiently dephosphorylate tau only when neither protein is bound to MTs. Depolymerization of MTs or dissociation of PP2A from MTs thus potentiates the phosphatase activity of PP2A for soluble tau.	bind
24070	6	7714	6	10	NULL	0	NULL	statement 2			inhibits					PP2A		catalytic activity of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_250	10464280	3) PP2A binds to tau and MTs through distinct sites and therefore might be able to anchor tau to MTs. 4) Since MTs and PP2A compete for binding to the same region on tau and binding of PP2A to MTs inhibits its catalytic activity, PP2A can efficiently dephosphorylate tau only when neither protein is bound to MTs. Depolymerization of MTs or dissociation of PP2A from MTs thus potentiates the phosphatase activity of PP2A for soluble tau.	bind
24072	7	7714	6	NULL	NULL	0	NULL	PP2A	NULL		dephosphorylate	NULL	efficiently			tau	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_250	10464280	3) PP2A binds to tau and MTs through distinct sites and therefore might be able to anchor tau to MTs. 4) Since MTs and PP2A compete for binding to the same region on tau and binding of PP2A to MTs inhibits its catalytic activity, PP2A can efficiently dephosphorylate tau only when neither protein is bound to MTs. Depolymerization of MTs or dissociation of PP2A from MTs thus potentiates the phosphatase activity of PP2A for soluble tau.	bind
24075	8	7714	6	NULL	NULL	0	NULL	statement 7	NULL		occurs under conditions of	NULL				tau	NULL	unbound			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_250	10464280	3) PP2A binds to tau and MTs through distinct sites and therefore might be able to anchor tau to MTs. 4) Since MTs and PP2A compete for binding to the same region on tau and binding of PP2A to MTs inhibits its catalytic activity, PP2A can efficiently dephosphorylate tau only when neither protein is bound to MTs. Depolymerization of MTs or dissociation of PP2A from MTs thus potentiates the phosphatase activity of PP2A for soluble tau.	bind
24076	9	7714	6	NULL	NULL	0	NULL	PP2A	NULL		exhibits	NULL				phosphatase activity	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_250	10464280	3) PP2A binds to tau and MTs through distinct sites and therefore might be able to anchor tau to MTs. 4) Since MTs and PP2A compete for binding to the same region on tau and binding of PP2A to MTs inhibits its catalytic activity, PP2A can efficiently dephosphorylate tau only when neither protein is bound to MTs. Depolymerization of MTs or dissociation of PP2A from MTs thus potentiates the phosphatase activity of PP2A for soluble tau.	bind
24077	10	7714	6	NULL	NULL	0	NULL	MT	NULL	depolymerization of 	potentiates	NULL				statement 9	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_250	10464280	3) PP2A binds to tau and MTs through distinct sites and therefore might be able to anchor tau to MTs. 4) Since MTs and PP2A compete for binding to the same region on tau and binding of PP2A to MTs inhibits its catalytic activity, PP2A can efficiently dephosphorylate tau only when neither protein is bound to MTs. Depolymerization of MTs or dissociation of PP2A from MTs thus potentiates the phosphatase activity of PP2A for soluble tau.	bind
24123	11	7714	6	NULL	NULL	0	NULL	PP2A	NULL		dissociates from	NULL				MT	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_250	10464280	3) PP2A binds to tau and MTs through distinct sites and therefore might be able to anchor tau to MTs. 4) Since MTs and PP2A compete for binding to the same region on tau and binding of PP2A to MTs inhibits its catalytic activity, PP2A can efficiently dephosphorylate tau only when neither protein is bound to MTs. Depolymerization of MTs or dissociation of PP2A from MTs thus potentiates the phosphatase activity of PP2A for soluble tau.	bind
24124	12	7714	6	NULL	NULL	0	NULL	statement 10	NULL		potentiates	NULL				statement 9	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_250	10464280	3) PP2A binds to tau and MTs through distinct sites and therefore might be able to anchor tau to MTs. 4) Since MTs and PP2A compete for binding to the same region on tau and binding of PP2A to MTs inhibits its catalytic activity, PP2A can efficiently dephosphorylate tau only when neither protein is bound to MTs. Depolymerization of MTs or dissociation of PP2A from MTs thus potentiates the phosphatase activity of PP2A for soluble tau.	bind
46763	13	7714	6	10	NULL	0	NULL	statement 7	NULL		occur under conditions of	NULL				PP2A	NULL	unbound			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_250	10464280	3) PP2A binds to tau and MTs through distinct sites and therefore might be able to anchor tau to MTs. 4) Since MTs and PP2A compete for binding to the same region on tau and binding of PP2A to MTs inhibits its catalytic activity, PP2A can efficiently dephosphorylate tau only when neither protein is bound to MTs. Depolymerization of MTs or dissociation of PP2A from MTs thus potentiates the phosphatase activity of PP2A for soluble tau.	bind
31115	1	7715	5	13	NULL	NULL	NULL	NTAB  fragments	GP	soluble 	bind					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_35355_s_251	9857078	3) Soluble fragments of NTAB bind to heparin better than LDL does.	bind
31116	2	7715	5	13	NULL	NULL	NULL	LDL	GP		bind					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_35355_s_251	9857078	3) Soluble fragments of NTAB bind to heparin better than LDL does.	bind
31117	3	7715	5	13	NULL	NULL	NULL	statement 1	Process		better than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_35355_s_251	9857078	3) Soluble fragments of NTAB bind to heparin better than LDL does.	bind
24125	1	7715	6	10	NULL	0	NULL	NTAB fragments	NULL	soluble	bind	NULL				heparin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_35355_s_251	9857078	3) Soluble fragments of NTAB bind to heparin better than LDL does.	bind
24126	2	7715	6	NULL	NULL	0	NULL	LDL	NULL		bind	NULL				heparin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_52_35355_s_251	9857078	3) Soluble fragments of NTAB bind to heparin better than LDL does.	bind
24127	3	7715	6	NULL	NULL	0	NULL	statement 1	NULL		is better than	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_52_35355_s_251	9857078	3) Soluble fragments of NTAB bind to heparin better than LDL does.	bind
31118	1	7716	5	13	NULL	NULL	NULL	PDI	GP		bind					TG	GP		Ser789-Met1178 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_3_1920_s_346	10636893	3) Surface plasmon resonance analysis of TG/PDI interaction characteristics indicated: (i) that PDI binds TG, but only in acidic conditions, and that it preferentially recognizes immature molecules, and (ii) that the Ser789-Met1178 domain is involved in binding, even if the cysteine-rich module is deleted.	bind
31119	2	7716	5	13	NULL	NULL	NULL	statement 1	Process		occurs in		only			acidic conditions					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_3_1920_s_346	10636893	3) Surface plasmon resonance analysis of TG/PDI interaction characteristics indicated: (i) that PDI binds TG, but only in acidic conditions, and that it preferentially recognizes immature molecules, and (ii) that the Ser789-Met1178 domain is involved in binding, even if the cysteine-rich module is deleted.	bind
31120	3	7716	5	13	NULL	NULL	NULL	PDI	GP		recognizes		preferentially			immature molecules	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_3_1920_s_346	10636893	3) Surface plasmon resonance analysis of TG/PDI interaction characteristics indicated: (i) that PDI binds TG, but only in acidic conditions, and that it preferentially recognizes immature molecules, and (ii) that the Ser789-Met1178 domain is involved in binding, even if the cysteine-rich module is deleted.	bind
31122	4	7716	5	13	NULL	NULL	NULL	statement 1	Process		absence of					TG	GP		cysteine-rich module		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_3_1920_s_346	10636893	3) Surface plasmon resonance analysis of TG/PDI interaction characteristics indicated: (i) that PDI binds TG, but only in acidic conditions, and that it preferentially recognizes immature molecules, and (ii) that the Ser789-Met1178 domain is involved in binding, even if the cysteine-rich module is deleted.	bind
24129	2	7716	6	NULL	NULL	0	NULL	statement 1	NULL		occurs in	NULL	only			acidic conditions	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_3_1920_s_346	10636893	3) Surface plasmon resonance analysis of TG/PDI interaction characteristics indicated: (i) that PDI binds TG, but only in acidic conditions, and that it preferentially recognizes immature molecules, and (ii) that the Ser789-Met1178 domain is involved in binding, even if the cysteine-rich module is deleted.	bind
24131	4	7716	6	NULL	NULL	0	NULL	statement 3	NULL		occurs even after	NULL					NULL	deletion of	cysteine-rich module		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_3_1920_s_346	10636893	3) Surface plasmon resonance analysis of TG/PDI interaction characteristics indicated: (i) that PDI binds TG, but only in acidic conditions, and that it preferentially recognizes immature molecules, and (ii) that the Ser789-Met1178 domain is involved in binding, even if the cysteine-rich module is deleted.	bind
46764	5	7716	6	10	NULL	0	NULL	PDI	NULL		recognizes	NULL	preferentially			immature molecules	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_3_1920_s_346	10636893	3) Surface plasmon resonance analysis of TG/PDI interaction characteristics indicated: (i) that PDI binds TG, but only in acidic conditions, and that it preferentially recognizes immature molecules, and (ii) that the Ser789-Met1178 domain is involved in binding, even if the cysteine-rich module is deleted.	bind
55544	1	7716	6	10	NULL	0	NULL	PDI			bind					TG			Ser789-Met1178 domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_3_1920_s_346	10636893	3) Surface plasmon resonance analysis of TG/PDI interaction characteristics indicated: (i) that PDI binds TG, but only in acidic conditions, and that it preferentially recognizes immature molecules, and (ii) that the Ser789-Met1178 domain is involved in binding, even if the cysteine-rich module is deleted.	bind
31130	1	7717	5	13	NULL	NULL	NULL	Synapsins	GP		bind					ADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_3_1425_s_157	9430678	3) Synapsins bind ADP with a much lower affinity than ATP, indicating that after hydrolysis, ADP would be exchanged for ATP.	bind
31131	2	7717	5	13	NULL	NULL	NULL	Synapsins	GP		bind					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_3_1425_s_157	9430678	3) Synapsins bind ADP with a much lower affinity than ATP, indicating that after hydrolysis, ADP would be exchanged for ATP.	bind
31133	3	7717	5	13	NULL	NULL	NULL	statement 1	Process		lower affinity than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_3_1425_s_157	9430678	3) Synapsins bind ADP with a much lower affinity than ATP, indicating that after hydrolysis, ADP would be exchanged for ATP.	bind
31134	4	7717	5	13	NULL	NULL	NULL	ADP	Chemical		is exchanged for					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_3_1425_s_157	9430678	3) Synapsins bind ADP with a much lower affinity than ATP, indicating that after hydrolysis, ADP would be exchanged for ATP.	bind
31136	5	7717	5	13	NULL	NULL	NULL	statement 4	Process		occurs after					hydrolysis	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_3_1425_s_157	9430678	3) Synapsins bind ADP with a much lower affinity than ATP, indicating that after hydrolysis, ADP would be exchanged for ATP.	bind
24132	1	7717	6	NULL	NULL	0	NULL	Synapsins	NULL		bind	NULL				ADP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_3_1425_s_157	9430678	3) Synapsins bind ADP with a much lower affinity than ATP, indicating that after hydrolysis, ADP would be exchanged for ATP.	bind
24133	2	7717	6	NULL	NULL	0	NULL	Synapsins	NULL		bind	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_3_1425_s_157	9430678	3) Synapsins bind ADP with a much lower affinity than ATP, indicating that after hydrolysis, ADP would be exchanged for ATP.	bind
24134	3	7717	6	10	NULL	0	NULL	statement 2	NULL		 lower affinity than	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_3_1425_s_157	9430678	3) Synapsins bind ADP with a much lower affinity than ATP, indicating that after hydrolysis, ADP would be exchanged for ATP.	bind
24135	4	7717	6	NULL	NULL	0	NULL	ADP	NULL		is exchanged for	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_3_1425_s_157	9430678	3) Synapsins bind ADP with a much lower affinity than ATP, indicating that after hydrolysis, ADP would be exchanged for ATP.	bind
24136	5	7717	6	NULL	NULL	0	NULL	statement 4	NULL		occurs after	NULL				hydrolysis	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_3_1425_s_157	9430678	3) Synapsins bind ADP with a much lower affinity than ATP, indicating that after hydrolysis, ADP would be exchanged for ATP.	bind
31137	1	7718	5	13	NULL	NULL	NULL	DnaK	GP		bind					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_11_6137_s_158	8626401	3) The absence of K   inhibits  DnaK's ATPase activity and conformational change but not the  binding of ATP to DnaK (Palleros  et al., 1993).	bind
44705	2	7718	5	13	NULL	NULL	NULL	DnaK	GP		exhibit					ATPase activity 	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_11_6137_s_158	8626401	3) The absence of K   inhibits  DnaK's ATPase activity and conformational change but not the  binding of ATP to DnaK (Palleros  et al., 1993).	bind
44706	4	7718	5	13	NULL	NULL	NULL			absence of	inhibit			K		DnaK	GP	conformational change of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_11_6137_s_158	8626401	3) The absence of K   inhibits  DnaK's ATPase activity and conformational change but not the  binding of ATP to DnaK (Palleros  et al., 1993).	bind
44707	5	7718	5	13	NULL	NULL	NULL			absence of	does not inhibit			K		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_11_6137_s_158	8626401	3) The absence of K   inhibits  DnaK's ATPase activity and conformational change but not the  binding of ATP to DnaK (Palleros  et al., 1993).	bind
46765	3	7718	5	13	NULL	NULL	NULL			absence of	inhibit			K		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_11_6137_s_158	8626401	3) The absence of K   inhibits  DnaK's ATPase activity and conformational change but not the  binding of ATP to DnaK (Palleros  et al., 1993).	bind
24137	1	7718	6	NULL	NULL	0	NULL	ATP	NULL		bind	NULL				DnaK	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_11_6137_s_158	8626401	3) The absence of K   inhibits  DnaK's ATPase activity and conformational change but not the  binding of ATP to DnaK (Palleros  et al., 1993).	bind
24138	2	7718	6	10	NULL	0	NULL	DnaK	NULL		exhibit	NULL				 ATPase activity	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_11_6137_s_158	8626401	3) The absence of K   inhibits  DnaK's ATPase activity and conformational change but not the  binding of ATP to DnaK (Palleros  et al., 1993).	bind
24139	3	7718	6	NULL	NULL	0	NULL		NULL	absence of	inhibits	NULL		K		Dnak	NULL	conformational change of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_11_6137_s_158	8626401	3) The absence of K   inhibits  DnaK's ATPase activity and conformational change but not the  binding of ATP to DnaK (Palleros  et al., 1993).	bind
24140	4	7718	6	NULL	NULL	0	NULL		NULL	absence of	does not inhibit	NULL		K		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_11_6137_s_158	8626401	3) The absence of K   inhibits  DnaK's ATPase activity and conformational change but not the  binding of ATP to DnaK (Palleros  et al., 1993).	bind
46766	5	7718	6	10	NULL	0	NULL		NULL	absence of	inhibit	NULL		K		statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_11_6137_s_158	8626401	3) The absence of K   inhibits  DnaK's ATPase activity and conformational change but not the  binding of ATP to DnaK (Palleros  et al., 1993).	bind
31140	1	7719	5	13	NULL	NULL	NULL	TCF	GP		is required in					bromocomplex	GP	formation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_7_5213_s_322	11083868	3) The DNA-dependent  in vitro interactions can be reconstituted on the Ets protein binding site E74, where Elk-1 binds in the absence of SRF, suggesting a sole requirement for TCF in bromocomplex formation.	bind
31354	2	7719	5	13	NULL	NULL	NULL	Elk-1	GP		bind									E74	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_7_5213_s_322	11083868	3) The DNA-dependent  in vitro interactions can be reconstituted on the Ets protein binding site E74, where Elk-1 binds in the absence of SRF, suggesting a sole requirement for TCF in bromocomplex formation.	bind
31355	3	7719	5	13	NULL	NULL	NULL	statement 2	Process		absence of					SRF	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_7_5213_s_322	11083868	3) The DNA-dependent  in vitro interactions can be reconstituted on the Ets protein binding site E74, where Elk-1 binds in the absence of SRF, suggesting a sole requirement for TCF in bromocomplex formation.	bind
31356	4	7719	5	13	NULL	NULL	NULL	E74	GP		is					Ets protein binding site	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_7_5213_s_322	11083868	3) The DNA-dependent  in vitro interactions can be reconstituted on the Ets protein binding site E74, where Elk-1 binds in the absence of SRF, suggesting a sole requirement for TCF in bromocomplex formation.	bind
24552	1	7719	6	NULL	NULL	0	NULL	TCF	NULL		plays a role in	NULL				bromocomplex	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_7_5213_s_322	11083868	3) The DNA-dependent  in vitro interactions can be reconstituted on the Ets protein binding site E74, where Elk-1 binds in the absence of SRF, suggesting a sole requirement for TCF in bromocomplex formation.	bind
24553	2	7719	6	NULL	NULL	0	NULL	Elk1	NULL	binding of	occurs in absence of	NULL				SRF	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_7_5213_s_322	11083868	3) The DNA-dependent  in vitro interactions can be reconstituted on the Ets protein binding site E74, where Elk-1 binds in the absence of SRF, suggesting a sole requirement for TCF in bromocomplex formation.	bind
24949	3	7719	6	10	NULL	0	NULL	Elk1	NULL		bind	NULL					NULL			 E74	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_7_5213_s_322	11083868	3) The DNA-dependent  in vitro interactions can be reconstituted on the Ets protein binding site E74, where Elk-1 binds in the absence of SRF, suggesting a sole requirement for TCF in bromocomplex formation.	bind
46767	4	7719	6	10	NULL	0	NULL	E74	NULL		is	NULL				Ets protein binding site	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_7_5213_s_322	11083868	3) The DNA-dependent  in vitro interactions can be reconstituted on the Ets protein binding site E74, where Elk-1 binds in the absence of SRF, suggesting a sole requirement for TCF in bromocomplex formation.	bind
31357	1	7721	5	13	NULL	NULL	NULL	insulin receptor	GP		bind					Hsp90	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_11_3071_s_33	9802897	3) The insulin receptor binds Hsp90, and antibodies to Hsp90 interfere with insulin signaling (Takata  et al., 1997  ).	bind
31358	2	7721	5	13	NULL	NULL	NULL	Hsp90 antibodies	GP		interfere with					insulin signaling	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_11_3071_s_33	9802897	3) The insulin receptor binds Hsp90, and antibodies to Hsp90 interfere with insulin signaling (Takata  et al., 1997  ).	bind
24143	1	7721	6	NULL	NULL	0	NULL	insulin receptor	NULL		bind	NULL				Hsp90	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_9_11_3071_s_33	9802897	3) The insulin receptor binds Hsp90, and antibodies to Hsp90 interfere with insulin signaling (Takata  et al., 1997  ).	bind
24144	2	7721	6	10	NULL	0	NULL	Hsp90 antibodies	NULL		interfere with	NULL				insulin signaling	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_11_3071_s_33	9802897	3) The insulin receptor binds Hsp90, and antibodies to Hsp90 interfere with insulin signaling (Takata  et al., 1997  ).	bind
31369	1	7722	5	13	NULL	NULL	NULL				bind			SH3 domain		linker	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_33_23776_s_282	16790421	3) The SH3 domain binds to the linker, which results in Src inactivation.	bind
31370	2	7722	5	13	NULL	NULL	NULL	statement 1	Process		results in					Src	GP	inactivation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_33_23776_s_282	16790421	3) The SH3 domain binds to the linker, which results in Src inactivation.	bind
24145	1	7722	6	NULL	NULL	0	NULL		NULL		bind	NULL		SH3 domain		linker	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_33_23776_s_282	16790421	3) The SH3 domain binds to the linker, which results in Src inactivation.	bind
24146	2	7722	6	NULL	NULL	0	NULL	statement 1	NULL		results in	NULL				src 	NULL	inactivation of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_33_23776_s_282	16790421	3) The SH3 domain binds to the linker, which results in Src inactivation.	bind
31371	1	7723	5	13	NULL	NULL	NULL	Taq	Organism		bind		might							GC-rich sequences	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_5694_s_216	12466277	3) The two polymerases might show significant differences in sequence specificity,  e.g. Taq might bind GC-rich sequences (more common in thermostable bacteria) tighter than mixed DNA sequences.	bind
31372	2	7723	5	13	NULL	NULL	NULL	statement 1	Process		occurs in		commonly			thermostable bacteria	Organism				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_5694_s_216	12466277	3) The two polymerases might show significant differences in sequence specificity,  e.g. Taq might bind GC-rich sequences (more common in thermostable bacteria) tighter than mixed DNA sequences.	bind
31373	3	7723	5	13	NULL	NULL	NULL	Taq	Organism		bind					DNA sequences	NucleicAcid	mixed			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_5694_s_216	12466277	3) The two polymerases might show significant differences in sequence specificity,  e.g. Taq might bind GC-rich sequences (more common in thermostable bacteria) tighter than mixed DNA sequences.	bind
31374	4	7723	5	13	NULL	NULL	NULL	statement 1	Process		tighter than					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_5694_s_216	12466277	3) The two polymerases might show significant differences in sequence specificity,  e.g. Taq might bind GC-rich sequences (more common in thermostable bacteria) tighter than mixed DNA sequences.	bind
24147	1	7723	6	NULL	NULL	0	NULL	Taq	NULL		bind	NULL	may				NULL			GC rich sequences	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_8_5694_s_216	12466277	3) The two polymerases might show significant differences in sequence specificity,  e.g. Taq might bind GC-rich sequences (more common in thermostable bacteria) tighter than mixed DNA sequences.	bind
24148	2	7723	6	10	NULL	0	NULL	Taq			bind		may			DNA sequences				mixed	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_5694_s_216	12466277	3) The two polymerases might show significant differences in sequence specificity,  e.g. Taq might bind GC-rich sequences (more common in thermostable bacteria) tighter than mixed DNA sequences.	bind
24149	3	7723	6	NULL	NULL	0	NULL	statement 1	NULL		is tighter than	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_8_5694_s_216	12466277	3) The two polymerases might show significant differences in sequence specificity,  e.g. Taq might bind GC-rich sequences (more common in thermostable bacteria) tighter than mixed DNA sequences.	bind
24150	4	7723	6	10	NULL	0	NULL	statement 1			occurs in		commonly			thermostable bacteria					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_5694_s_216	12466277	3) The two polymerases might show significant differences in sequence specificity,  e.g. Taq might bind GC-rich sequences (more common in thermostable bacteria) tighter than mixed DNA sequences.	bind
31375	1	7724	5	13	NULL	NULL	NULL	gp43	GP		bind			C terminus		gp45	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_39340_s_288	11504721	3) The x-ray crystal structure of the C terminus of gp43 bound to gp45 yielded a stoichiometry of 1 peptide per gp45 trimer ( 22), whereas fluorescence measurements in solution yielded a stoichiometry of 1 peptide per gp45 monomer ( 32).	bind
24151	1	7724	6	NULL	NULL	0	NULL	gp43	NULL		bind	NULL		C terminus		gp45	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_39340_s_288	11504721	3) The x-ray crystal structure of the C terminus of gp43 bound to gp45 yielded a stoichiometry of 1 peptide per gp45 trimer ( 22), whereas fluorescence measurements in solution yielded a stoichiometry of 1 peptide per gp45 monomer ( 32).	bind
31376	1	7725	5	13	NULL	NULL	NULL	pro-uPA	GP		bind					tumor cell receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_15_14899_s_8	14747469	3) Tumor cell receptor-bound pro-uPA could be efficiently cleaved by matriptase to generate enzymatically active two-chain uPA.	bind
31377	2	7725	5	13	NULL	NULL	NULL	matriptase	GP		cleaves		efficiently			statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_15_14899_s_8	14747469	3) Tumor cell receptor-bound pro-uPA could be efficiently cleaved by matriptase to generate enzymatically active two-chain uPA.	bind
31378	3	7725	5	13	NULL	NULL	NULL	statement 2	Process		generates					two-chain uPA	GP	enzymatically active			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_15_14899_s_8	14747469	3) Tumor cell receptor-bound pro-uPA could be efficiently cleaved by matriptase to generate enzymatically active two-chain uPA.	bind
24152	1	7725	6	NULL	NULL	0	NULL	Tumor cell receptor	NULL		bind	NULL				pro-uPA	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_15_14899_s_8	14747469	3) Tumor cell receptor-bound pro-uPA could be efficiently cleaved by matriptase to generate enzymatically active two-chain uPA.	bind
24153	2	7725	6	10	NULL	0	NULL	statement 1			is cleaved by		efficiently			matriptase					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_15_14899_s_8	14747469	3) Tumor cell receptor-bound pro-uPA could be efficiently cleaved by matriptase to generate enzymatically active two-chain uPA.	bind
46770	3	7725	6	10	NULL	0	NULL	statement 2	NULL		generates	NULL				two-chain uPA	NULL	enzymatically active			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_15_14899_s_8	14747469	3) Tumor cell receptor-bound pro-uPA could be efficiently cleaved by matriptase to generate enzymatically active two-chain uPA.	bind
31379	1	7726	5	13	NULL	NULL	NULL	intersectin	GP		bind		specifically			SCAMP1	GP		N-terminal NPF repeats		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_17_12752_s_162	10777571	3) Two proteins with a known function in clathrin coats are specifically bound to the N-terminal NPF repeats of SCAMP1, namely intersectin and gamma-synergin.	bind
31380	2	7726	5	13	NULL	NULL	NULL	gamma-synergin	GP		bind		specifically			SCAMP1	GP		N-terminal NPF repeats		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_17_12752_s_162	10777571	3) Two proteins with a known function in clathrin coats are specifically bound to the N-terminal NPF repeats of SCAMP1, namely intersectin and gamma-synergin.	bind
46771	3	7726	5	13	NULL	NULL	NULL	intersectin 	GP		function in					clathrin coats	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_17_12752_s_162	10777571	3) Two proteins with a known function in clathrin coats are specifically bound to the N-terminal NPF repeats of SCAMP1, namely intersectin and gamma-synergin.	bind
46772	4	7726	5	13	NULL	NULL	NULL	gamma-synergin	GP		function in					clathrin coats	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_17_12752_s_162	10777571	3) Two proteins with a known function in clathrin coats are specifically bound to the N-terminal NPF repeats of SCAMP1, namely intersectin and gamma-synergin.	bind
24154	1	7726	6	10	NULL	0	NULL	intersectin			bind		specifically			SCAMP1			N-terminal NPF repeats		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_17_12752_s_162	10777571	3) Two proteins with a known function in clathrin coats are specifically bound to the N-terminal NPF repeats of SCAMP1, namely intersectin and gamma-synergin.	bind
24155	2	7726	6	10	NULL	0	NULL	gamma-synergin			bind		specifically			SCAMP1			N-terminal NPF repeats		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_17_12752_s_162	10777571	3) Two proteins with a known function in clathrin coats are specifically bound to the N-terminal NPF repeats of SCAMP1, namely intersectin and gamma-synergin.	bind
24156	3	7726	6	NULL	NULL	0	NULL	intersectin	NULL		function in	NULL				clathrin coats	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_17_12752_s_162	10777571	3) Two proteins with a known function in clathrin coats are specifically bound to the N-terminal NPF repeats of SCAMP1, namely intersectin and gamma-synergin.	bind
24157	4	7726	6	NULL	NULL	0	NULL	gamma-synergin	NULL		function in	NULL				clathrin coats	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_17_12752_s_162	10777571	3) Two proteins with a known function in clathrin coats are specifically bound to the N-terminal NPF repeats of SCAMP1, namely intersectin and gamma-synergin.	bind
31381	1	7727	5	13	NULL	NULL	NULL	Ras	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_25157_s_248	11274179	3) Vincristine and paclitaxel have been shown to stimulate Ras binding to GTP, one of the avenues leading to activation of JNK/SAPK pathway ( 47), whereas our current data indicate that nocodazole activates Raf-1 through a Ras-independent mechanism.	bind
31382	2	7727	5	13	NULL	NULL	NULL	vincristine	Chemical		stimulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_25157_s_248	11274179	3) Vincristine and paclitaxel have been shown to stimulate Ras binding to GTP, one of the avenues leading to activation of JNK/SAPK pathway ( 47), whereas our current data indicate that nocodazole activates Raf-1 through a Ras-independent mechanism.	bind
31383	3	7727	5	13	NULL	NULL	NULL	paclitaxel	Chemical		stimulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_25157_s_248	11274179	3) Vincristine and paclitaxel have been shown to stimulate Ras binding to GTP, one of the avenues leading to activation of JNK/SAPK pathway ( 47), whereas our current data indicate that nocodazole activates Raf-1 through a Ras-independent mechanism.	bind
31384	4	7727	5	13	NULL	NULL	NULL	statement 1	Process		leads to					JNK/SAPK pathway	Process	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_25157_s_248	11274179	3) Vincristine and paclitaxel have been shown to stimulate Ras binding to GTP, one of the avenues leading to activation of JNK/SAPK pathway ( 47), whereas our current data indicate that nocodazole activates Raf-1 through a Ras-independent mechanism.	bind
31385	5	7727	5	13	NULL	NULL	NULL	nocodazole	Chemical		activates					Raf-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_25157_s_248	11274179	3) Vincristine and paclitaxel have been shown to stimulate Ras binding to GTP, one of the avenues leading to activation of JNK/SAPK pathway ( 47), whereas our current data indicate that nocodazole activates Raf-1 through a Ras-independent mechanism.	bind
31386	6	7727	5	13	NULL	NULL	NULL	statement 5	Process		is independent of					Ras	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_25157_s_248	11274179	3) Vincristine and paclitaxel have been shown to stimulate Ras binding to GTP, one of the avenues leading to activation of JNK/SAPK pathway ( 47), whereas our current data indicate that nocodazole activates Raf-1 through a Ras-independent mechanism.	bind
24158	1	7727	6	NULL	NULL	0	NULL	Ras	NULL		bind	NULL				GTP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_27_25157_s_248	11274179	3) Vincristine and paclitaxel have been shown to stimulate Ras binding to GTP, one of the avenues leading to activation of JNK/SAPK pathway ( 47), whereas our current data indicate that nocodazole activates Raf-1 through a Ras-independent mechanism.	bind
24159	2	7727	6	NULL	NULL	0	NULL	Vincristine	NULL		stimulates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_27_25157_s_248	11274179	3) Vincristine and paclitaxel have been shown to stimulate Ras binding to GTP, one of the avenues leading to activation of JNK/SAPK pathway ( 47), whereas our current data indicate that nocodazole activates Raf-1 through a Ras-independent mechanism.	bind
24160	3	7727	6	NULL	NULL	0	NULL	paclitaxel	NULL		stimulates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_27_25157_s_248	11274179	3) Vincristine and paclitaxel have been shown to stimulate Ras binding to GTP, one of the avenues leading to activation of JNK/SAPK pathway ( 47), whereas our current data indicate that nocodazole activates Raf-1 through a Ras-independent mechanism.	bind
24161	4	7727	6	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				JNK/SAPK pathway	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_27_25157_s_248	11274179	3) Vincristine and paclitaxel have been shown to stimulate Ras binding to GTP, one of the avenues leading to activation of JNK/SAPK pathway ( 47), whereas our current data indicate that nocodazole activates Raf-1 through a Ras-independent mechanism.	bind
24162	5	7727	6	NULL	NULL	0	NULL	Nocodazole	NULL		activates	NULL				Raf-1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_27_25157_s_248	11274179	3) Vincristine and paclitaxel have been shown to stimulate Ras binding to GTP, one of the avenues leading to activation of JNK/SAPK pathway ( 47), whereas our current data indicate that nocodazole activates Raf-1 through a Ras-independent mechanism.	bind
24163	6	7727	6	NULL	NULL	0	NULL	statement 5	NULL		is independent of	NULL				ras	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_27_25157_s_248	11274179	3) Vincristine and paclitaxel have been shown to stimulate Ras binding to GTP, one of the avenues leading to activation of JNK/SAPK pathway ( 47), whereas our current data indicate that nocodazole activates Raf-1 through a Ras-independent mechanism.	bind
31387	2	7728	5	13	NULL	NULL	NULL	LDL-c	GP		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_1_90_s_18	12524230	3, 4 LDL-c binds to the LDLR expressed on the surface of hepatocytes and is removed from the circulation by LDLR-mediated endocytosis.	bind
31388	4	7728	5	13	NULL	NULL	NULL	statement 3	Process		removes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_1_90_s_18	12524230	3, 4 LDL-c binds to the LDLR expressed on the surface of hepatocytes and is removed from the circulation by LDLR-mediated endocytosis.	bind
31389	3	7728	5	13	NULL	NULL	NULL	LDLR	GP		mediates					endocytosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_1_90_s_18	12524230	3, 4 LDL-c binds to the LDLR expressed on the surface of hepatocytes and is removed from the circulation by LDLR-mediated endocytosis.	bind
46773	1	7728	5	13	NULL	NULL	NULL	LDLR	GP		is expressed on					hepatocytes	Cell	surface of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_1_90_s_18	12524230	3, 4 LDL-c binds to the LDLR expressed on the surface of hepatocytes and is removed from the circulation by LDLR-mediated endocytosis.	bind
24164	2	7728	6	10	NULL	0	NULL	LDL-c 	NULL		bind	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_1_90_s_18	12524230	3, 4 LDL-c binds to the LDLR expressed on the surface of hepatocytes and is removed from the circulation by LDLR-mediated endocytosis.	bind
24166	1	7728	6	10	NULL	0	NULL	LDLR	NULL		is expressed on	NULL				hepatocytes	NULL	surface of 			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_1_90_s_18	12524230	3, 4 LDL-c binds to the LDLR expressed on the surface of hepatocytes and is removed from the circulation by LDLR-mediated endocytosis.	bind
24167	3	7728	6	10	NULL	0	NULL	LDLR	NULL		mediates	NULL				endocytosis	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_1_90_s_18	12524230	3, 4 LDL-c binds to the LDLR expressed on the surface of hepatocytes and is removed from the circulation by LDLR-mediated endocytosis.	bind
24168	4	7728	6	10	NULL	0	NULL	statement 2	NULL		is removed by	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_1_90_s_18	12524230	3, 4 LDL-c binds to the LDLR expressed on the surface of hepatocytes and is removed from the circulation by LDLR-mediated endocytosis.	bind
31390	1	7729	5	13	NULL	NULL	NULL	BAFF/BLyS receptor 3	GP		bind			surface loop		BAFF ligand 	GP				NULL		NULL	NULL	NULL	NULL	gw70_nature_431_7007_456_s_207	15361883	3, 958 965 (2002) |  Article |  PubMed |  ISI |  ChemPort |                    Kayagaki, N.  et al. BAFF/BLyS receptor 3 binds the B cell survival factor BAFF ligand through a discrete  surface loop and promotes processing of NF-kappaB2.	bind
31391	2	7729	5	13	NULL	NULL	NULL	statement 1	Process		promote					NF-kappaB2	GP	processing of			NULL		NULL	NULL	NULL	NULL	gw70_nature_431_7007_456_s_207	15361883	3, 958 965 (2002) |  Article |  PubMed |  ISI |  ChemPort |                    Kayagaki, N.  et al. BAFF/BLyS receptor 3 binds the B cell survival factor BAFF ligand through a discrete  surface loop and promotes processing of NF-kappaB2.	bind
46774	3	7729	5	13	NULL	NULL	NULL	BAFF ligand	GP		is a type of					B cell survival factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_nature_431_7007_456_s_207	15361883	3, 958 965 (2002) |  Article |  PubMed |  ISI |  ChemPort |                    Kayagaki, N.  et al. BAFF/BLyS receptor 3 binds the B cell survival factor BAFF ligand through a discrete  surface loop and promotes processing of NF-kappaB2.	bind
24169	1	7729	6	13	NULL	NULL	NULL	BAFF/BLyS receptor 3	GP		bind					 BAFF ligand	GP				NULL		NULL	NULL	NULL	NULL	gw70_nature_431_7007_456_s_207	15361883	3, 958 965 (2002) |  Article |  PubMed |  ISI |  ChemPort |                    Kayagaki, N.  et al. BAFF/BLyS receptor 3 binds the B cell survival factor BAFF ligand through a discrete  surface loop and promotes processing of NF-kappaB2.	bind
24170	2	7729	6	NULL	NULL	0	NULL	statement 1	NULL		occurs through	NULL				surface loop	NULL	discrete			NULL		0	NULL	NULL	NULL	gw70_nature_431_7007_456_s_207	15361883	3, 958 965 (2002) |  Article |  PubMed |  ISI |  ChemPort |                    Kayagaki, N.  et al. BAFF/BLyS receptor 3 binds the B cell survival factor BAFF ligand through a discrete  surface loop and promotes processing of NF-kappaB2.	bind
24171	3	7729	6	NULL	NULL	0	NULL	statement 1	NULL		promotes	NULL				NF-kappaB2	NULL	processing of			NULL		0	NULL	NULL	NULL	gw70_nature_431_7007_456_s_207	15361883	3, 958 965 (2002) |  Article |  PubMed |  ISI |  ChemPort |                    Kayagaki, N.  et al. BAFF/BLyS receptor 3 binds the B cell survival factor BAFF ligand through a discrete  surface loop and promotes processing of NF-kappaB2.	bind
46775	4	7729	6	10	NULL	0	NULL	BAFF ligand	NULL		is a type of	NULL				B cell survival factor	NULL				NULL		0	NULL	NULL	NULL	gw70_nature_431_7007_456_s_207	15361883	3, 958 965 (2002) |  Article |  PubMed |  ISI |  ChemPort |                    Kayagaki, N.  et al. BAFF/BLyS receptor 3 binds the B cell survival factor BAFF ligand through a discrete  surface loop and promotes processing of NF-kappaB2.	bind
31392	1	7730	5	13	NULL	NULL	NULL	Hop	GP		bind					hsp90	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_41_38294_s_380	12161444	3, Hop that is bound to hsp90 binds to hsp70-ADP.	bind
31393	2	7730	5	13	NULL	NULL	NULL	statement 1	GP		bind					hsp70-ADP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_41_38294_s_380	12161444	3, Hop that is bound to hsp90 binds to hsp70-ADP.	bind
24211	1	7730	6	NULL	NULL	0	NULL	Hop	NULL		bind	NULL				hsp90	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_41_38294_s_380	12161444	3, Hop that is bound to hsp90 binds to hsp70-ADP.	bind
24212	2	7730	6	10	NULL	0	NULL	statement 1			bind					hsp70-ADP					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_41_38294_s_380	12161444	3, Hop that is bound to hsp90 binds to hsp70-ADP.	bind
31561	1	7731	5	13	NULL	NULL	NULL	T complex	GP		associates with					cellular factors	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_54_0_187_s_347	11018128	3, T complex associates with cellular factors; VirD2 binds to AtKAP  ( 3a) and cyclophilins ( 3b), VirE2 binds to VIP1 and/or VIP2 ( 3c), the VirD2 NLS region is phosphorylated ( 3d), and AtKAP  may interact with the putative AtKAPbeta ( 3e).	bind
31562	2	7731	5	13	NULL	NULL	NULL	VirD2	GP		bind					AtKAP	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_54_0_187_s_347	11018128	3, T complex associates with cellular factors; VirD2 binds to AtKAP  ( 3a) and cyclophilins ( 3b), VirE2 binds to VIP1 and/or VIP2 ( 3c), the VirD2 NLS region is phosphorylated ( 3d), and AtKAP  may interact with the putative AtKAPbeta ( 3e).	bind
31563	3	7731	5	13	NULL	NULL	NULL	VirD2	GP		bind					cyclophilins	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_54_0_187_s_347	11018128	3, T complex associates with cellular factors; VirD2 binds to AtKAP  ( 3a) and cyclophilins ( 3b), VirE2 binds to VIP1 and/or VIP2 ( 3c), the VirD2 NLS region is phosphorylated ( 3d), and AtKAP  may interact with the putative AtKAPbeta ( 3e).	bind
31564	4	7731	5	13	NULL	NULL	NULL	VirE2	GP		bind					VIP1	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_54_0_187_s_347	11018128	3, T complex associates with cellular factors; VirD2 binds to AtKAP  ( 3a) and cyclophilins ( 3b), VirE2 binds to VIP1 and/or VIP2 ( 3c), the VirD2 NLS region is phosphorylated ( 3d), and AtKAP  may interact with the putative AtKAPbeta ( 3e).	bind
31565	5	7731	5	13	NULL	NULL	NULL	VirE2	GP		bind					VIP2	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_54_0_187_s_347	11018128	3, T complex associates with cellular factors; VirD2 binds to AtKAP  ( 3a) and cyclophilins ( 3b), VirE2 binds to VIP1 and/or VIP2 ( 3c), the VirD2 NLS region is phosphorylated ( 3d), and AtKAP  may interact with the putative AtKAPbeta ( 3e).	bind
31566	6	7731	5	13	NULL	NULL	NULL	statement 4	Process		is alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_54_0_187_s_347	11018128	3, T complex associates with cellular factors; VirD2 binds to AtKAP  ( 3a) and cyclophilins ( 3b), VirE2 binds to VIP1 and/or VIP2 ( 3c), the VirD2 NLS region is phosphorylated ( 3d), and AtKAP  may interact with the putative AtKAPbeta ( 3e).	bind
31567	7	7731	5	13	NULL	NULL	NULL	VirD2	GP		undergoes			NLS		phosphorylation	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_54_0_187_s_347	11018128	3, T complex associates with cellular factors; VirD2 binds to AtKAP  ( 3a) and cyclophilins ( 3b), VirE2 binds to VIP1 and/or VIP2 ( 3c), the VirD2 NLS region is phosphorylated ( 3d), and AtKAP  may interact with the putative AtKAPbeta ( 3e).	bind
31568	8	7731	5	13	NULL	NULL	NULL	AtKAP	GP		interacts with		may			AtKAPbeta	GP	putative			NULL		NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_54_0_187_s_347	11018128	3, T complex associates with cellular factors; VirD2 binds to AtKAP  ( 3a) and cyclophilins ( 3b), VirE2 binds to VIP1 and/or VIP2 ( 3c), the VirD2 NLS region is phosphorylated ( 3d), and AtKAP  may interact with the putative AtKAPbeta ( 3e).	bind
24213	1	7731	6	NULL	NULL	0	NULL	VirE2	NULL		bind	NULL				VIP1	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_54_0_187_s_347	11018128	3, T complex associates with cellular factors; VirD2 binds to AtKAP  ( 3a) and cyclophilins ( 3b), VirE2 binds to VIP1 and/or VIP2 ( 3c), the VirD2 NLS region is phosphorylated ( 3d), and AtKAP  may interact with the putative AtKAPbeta ( 3e).	bind
24214	2	7731	6	NULL	NULL	0	NULL	VirE2	NULL		bind	NULL				VIP2	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_54_0_187_s_347	11018128	3, T complex associates with cellular factors; VirD2 binds to AtKAP  ( 3a) and cyclophilins ( 3b), VirE2 binds to VIP1 and/or VIP2 ( 3c), the VirD2 NLS region is phosphorylated ( 3d), and AtKAP  may interact with the putative AtKAPbeta ( 3e).	bind
24215	3	7731	6	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_54_0_187_s_347	11018128	3, T complex associates with cellular factors; VirD2 binds to AtKAP  ( 3a) and cyclophilins ( 3b), VirE2 binds to VIP1 and/or VIP2 ( 3c), the VirD2 NLS region is phosphorylated ( 3d), and AtKAP  may interact with the putative AtKAPbeta ( 3e).	bind
24216	4	7731	6	NULL	NULL	0	NULL	VirD2	NULL		bind	NULL				AtKAP	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_54_0_187_s_347	11018128	3, T complex associates with cellular factors; VirD2 binds to AtKAP  ( 3a) and cyclophilins ( 3b), VirE2 binds to VIP1 and/or VIP2 ( 3c), the VirD2 NLS region is phosphorylated ( 3d), and AtKAP  may interact with the putative AtKAPbeta ( 3e).	bind
24234	5	7731	6	10	NULL	0	NULL	VirD2	NULL		undergoes	NULL		NLS		phosphorylation	NULL				NULL		NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_54_0_187_s_347	11018128	3, T complex associates with cellular factors; VirD2 binds to AtKAP  ( 3a) and cyclophilins ( 3b), VirE2 binds to VIP1 and/or VIP2 ( 3c), the VirD2 NLS region is phosphorylated ( 3d), and AtKAP  may interact with the putative AtKAPbeta ( 3e).	bind
24235	6	7731	6	NULL	NULL	0	NULL	AtKAP	NULL		interact with	NULL	may			AtKAPbeta	NULL	putative			NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_54_0_187_s_347	11018128	3, T complex associates with cellular factors; VirD2 binds to AtKAP  ( 3a) and cyclophilins ( 3b), VirE2 binds to VIP1 and/or VIP2 ( 3c), the VirD2 NLS region is phosphorylated ( 3d), and AtKAP  may interact with the putative AtKAPbeta ( 3e).	bind
46776	7	7731	6	10	NULL	0	NULL	T complex	NULL		associate with	NULL				cellular factors	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_54_0_187_s_347	11018128	3, T complex associates with cellular factors; VirD2 binds to AtKAP  ( 3a) and cyclophilins ( 3b), VirE2 binds to VIP1 and/or VIP2 ( 3c), the VirD2 NLS region is phosphorylated ( 3d), and AtKAP  may interact with the putative AtKAPbeta ( 3e).	bind
46777	8	7731	6	10	NULL	0	NULL	VirD2	NULL		bind	NULL				cyclophilins	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_54_0_187_s_347	11018128	3, T complex associates with cellular factors; VirD2 binds to AtKAP  ( 3a) and cyclophilins ( 3b), VirE2 binds to VIP1 and/or VIP2 ( 3c), the VirD2 NLS region is phosphorylated ( 3d), and AtKAP  may interact with the putative AtKAPbeta ( 3e).	bind
31569	1	7733	5	13	NULL	NULL	NULL				bind			C domain		actin monomer	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_15_10589_s_277	16403731	3, the C domain then binds the actin monomer and, with the WH2 domain, positions it  on the Arp2/3 complex.	bind
24236	1	7733	6	NULL	NULL	0	NULL		NULL		bind	NULL		C domain		actin monomer	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_15_10589_s_277	16403731	3, the C domain then binds the actin monomer and, with the WH2 domain, positions it  on the Arp2/3 complex.	bind
31572	1	7735	5	13	NULL	NULL	NULL	s-FasL	GP		bind					Fas (APO-1/CD95) receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_6_1947_s_17	9846984	3- 5  Both tm- and s-FasL bind to the Fas (APO-1/CD95) receptor and induce apoptosis.	bind
31573	2	7735	5	13	NULL	NULL	NULL	statement 1	Process		induces					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_6_1947_s_17	9846984	3- 5  Both tm- and s-FasL bind to the Fas (APO-1/CD95) receptor and induce apoptosis.	bind
31575	3	7735	5	13	NULL	NULL	NULL	tm-FasL	GP		bind					Fas (APO-1/CD95) receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_6_1947_s_17	9846984	3- 5  Both tm- and s-FasL bind to the Fas (APO-1/CD95) receptor and induce apoptosis.	bind
31577	4	7735	5	13	NULL	NULL	NULL	statement 3	Process		induces					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_6_1947_s_17	9846984	3- 5  Both tm- and s-FasL bind to the Fas (APO-1/CD95) receptor and induce apoptosis.	bind
24237	1	7735	6	NULL	NULL	0	NULL	tm-FasL	NULL		bind	NULL				Fas (APO-1/CD95) receptor	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_6_1947_s_17	9846984	3- 5  Both tm- and s-FasL bind to the Fas (APO-1/CD95) receptor and induce apoptosis.	bind
24554	2	7735	6	NULL	NULL	0	NULL	s-FasL	NULL		bind	NULL				Fas (APO-1/CD95) receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_6_1947_s_17	9846984	3- 5  Both tm- and s-FasL bind to the Fas (APO-1/CD95) receptor and induce apoptosis.	bind
24555	3	7735	6	NULL	NULL	0	NULL	statement 1	NULL		induce	NULL				apoptosis	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_6_1947_s_17	9846984	3- 5  Both tm- and s-FasL bind to the Fas (APO-1/CD95) receptor and induce apoptosis.	bind
24556	4	7735	6	NULL	NULL	0	NULL	statement 2	NULL		induce	NULL				apoptosis	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_6_1947_s_17	9846984	3- 5  Both tm- and s-FasL bind to the Fas (APO-1/CD95) receptor and induce apoptosis.	bind
31578	1	7737	5	13	NULL	NULL	NULL	3-Hydroxyphthaloyl lg	GP		bind					HSV-1 virus particles	Organism				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1482_1_327_s_136	11058773	3-Hydroxyphthaloyl  lg binds to HSV-1, HSV-2 and HCMV virus particles and inhibits their binding of anti-glycoprotein E and anti-gC monoclonal antibodies.	bind
31581	2	7737	5	13	NULL	NULL	NULL	3-Hydroxyphthaloyl lg	GP		bind					HSV-2 virus particles	Organism				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1482_1_327_s_136	11058773	3-Hydroxyphthaloyl  lg binds to HSV-1, HSV-2 and HCMV virus particles and inhibits their binding of anti-glycoprotein E and anti-gC monoclonal antibodies.	bind
31582	3	7737	5	13	NULL	NULL	NULL	3-Hydroxyphthaloyl lg	GP		bind					HCMV virus particles	Organism				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1482_1_327_s_136	11058773	3-Hydroxyphthaloyl  lg binds to HSV-1, HSV-2 and HCMV virus particles and inhibits their binding of anti-glycoprotein E and anti-gC monoclonal antibodies.	bind
31593	4	7737	5	13	NULL	NULL	NULL	HSV-1 virus particles	Organism		bind					anti-glycoprotein E	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1482_1_327_s_136	11058773	3-Hydroxyphthaloyl  lg binds to HSV-1, HSV-2 and HCMV virus particles and inhibits their binding of anti-glycoprotein E and anti-gC monoclonal antibodies.	bind
31594	5	7737	5	13	NULL	NULL	NULL	HSV-2 virus particles	Organism		bind					anti-glycoprotein E	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1482_1_327_s_136	11058773	3-Hydroxyphthaloyl  lg binds to HSV-1, HSV-2 and HCMV virus particles and inhibits their binding of anti-glycoprotein E and anti-gC monoclonal antibodies.	bind
31595	6	7737	5	13	NULL	NULL	NULL	HCMV virus particles	Organism		bind					anti-glycoprotein E	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1482_1_327_s_136	11058773	3-Hydroxyphthaloyl  lg binds to HSV-1, HSV-2 and HCMV virus particles and inhibits their binding of anti-glycoprotein E and anti-gC monoclonal antibodies.	bind
31598	7	7737	5	13	NULL	NULL	NULL	statement 1	Process		inhibits					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1482_1_327_s_136	11058773	3-Hydroxyphthaloyl  lg binds to HSV-1, HSV-2 and HCMV virus particles and inhibits their binding of anti-glycoprotein E and anti-gC monoclonal antibodies.	bind
31610	8	7737	5	13	NULL	NULL	NULL	statement 2	Process		inhibits					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1482_1_327_s_136	11058773	3-Hydroxyphthaloyl  lg binds to HSV-1, HSV-2 and HCMV virus particles and inhibits their binding of anti-glycoprotein E and anti-gC monoclonal antibodies.	bind
31611	9	7737	5	13	NULL	NULL	NULL	statement 3	Process		inhibits					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1482_1_327_s_136	11058773	3-Hydroxyphthaloyl  lg binds to HSV-1, HSV-2 and HCMV virus particles and inhibits their binding of anti-glycoprotein E and anti-gC monoclonal antibodies.	bind
31612	10	7737	5	13	NULL	NULL	NULL	HSV-1 virus particles	Organism		bind					anti-gC monoclonal antibodies	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1482_1_327_s_136	11058773	3-Hydroxyphthaloyl  lg binds to HSV-1, HSV-2 and HCMV virus particles and inhibits their binding of anti-glycoprotein E and anti-gC monoclonal antibodies.	bind
31613	11	7737	5	13	NULL	NULL	NULL	HSV-2 virus particles	Organism		bind					anti-gC monoclonal antibodies	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1482_1_327_s_136	11058773	3-Hydroxyphthaloyl  lg binds to HSV-1, HSV-2 and HCMV virus particles and inhibits their binding of anti-glycoprotein E and anti-gC monoclonal antibodies.	bind
31614	12	7737	5	13	NULL	NULL	NULL	HCMV virus particles	Organism		bind					anti-gC monoclonal antibodies	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1482_1_327_s_136	11058773	3-Hydroxyphthaloyl  lg binds to HSV-1, HSV-2 and HCMV virus particles and inhibits their binding of anti-glycoprotein E and anti-gC monoclonal antibodies.	bind
31615	13	7737	5	13	NULL	NULL	NULL	statement 1	Process		inhibits					statement 10	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1482_1_327_s_136	11058773	3-Hydroxyphthaloyl  lg binds to HSV-1, HSV-2 and HCMV virus particles and inhibits their binding of anti-glycoprotein E and anti-gC monoclonal antibodies.	bind
31616	14	7737	5	13	NULL	NULL	NULL	statement 2	Process		inhibits					statement 11	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1482_1_327_s_136	11058773	3-Hydroxyphthaloyl  lg binds to HSV-1, HSV-2 and HCMV virus particles and inhibits their binding of anti-glycoprotein E and anti-gC monoclonal antibodies.	bind
31617	15	7737	5	13	NULL	NULL	NULL	statement 3	Process		inhibits					statement 12	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1482_1_327_s_136	11058773	3-Hydroxyphthaloyl  lg binds to HSV-1, HSV-2 and HCMV virus particles and inhibits their binding of anti-glycoprotein E and anti-gC monoclonal antibodies.	bind
24238	1	7737	6	NULL	NULL	0	NULL	Hydroxyphthaloyl lg	NULL		bind	NULL				HSV-1	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1482_1_327_s_136	11058773	3-Hydroxyphthaloyl  lg binds to HSV-1, HSV-2 and HCMV virus particles and inhibits their binding of anti-glycoprotein E and anti-gC monoclonal antibodies.	bind
24239	2	7737	6	NULL	NULL	0	NULL	Hydroxyphthaloyl lg	NULL		bind	NULL				HSV-2	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1482_1_327_s_136	11058773	3-Hydroxyphthaloyl  lg binds to HSV-1, HSV-2 and HCMV virus particles and inhibits their binding of anti-glycoprotein E and anti-gC monoclonal antibodies.	bind
24240	3	7737	6	NULL	NULL	0	NULL	Hydroxyphthaloyl lg	NULL		bind	NULL				HCMV virus particles	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1482_1_327_s_136	11058773	3-Hydroxyphthaloyl  lg binds to HSV-1, HSV-2 and HCMV virus particles and inhibits their binding of anti-glycoprotein E and anti-gC monoclonal antibodies.	bind
24557	4	7737	6	NULL	NULL	0	NULL	HSV-1	NULL		bind	NULL				anti-glycoprotein E monoclonal antibody	NULL				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1482_1_327_s_136	11058773	3-Hydroxyphthaloyl  lg binds to HSV-1, HSV-2 and HCMV virus particles and inhibits their binding of anti-glycoprotein E and anti-gC monoclonal antibodies.	bind
24558	5	7737	6	NULL	NULL	0	NULL	HSV-2	NULL		bind	NULL				anti-glycoprotein E monoclonal antibody	NULL				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1482_1_327_s_136	11058773	3-Hydroxyphthaloyl  lg binds to HSV-1, HSV-2 and HCMV virus particles and inhibits their binding of anti-glycoprotein E and anti-gC monoclonal antibodies.	bind
24559	6	7737	6	NULL	NULL	0	NULL	HCMV	NULL		bind	NULL				anti-glycoprotein E monoclonal antibody	NULL				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1482_1_327_s_136	11058773	3-Hydroxyphthaloyl  lg binds to HSV-1, HSV-2 and HCMV virus particles and inhibits their binding of anti-glycoprotein E and anti-gC monoclonal antibodies.	bind
24560	7	7737	6	NULL	NULL	0	NULL	HSV-1	NULL		bind	NULL				anti-gC monoclonal antibody	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1482_1_327_s_136	11058773	3-Hydroxyphthaloyl  lg binds to HSV-1, HSV-2 and HCMV virus particles and inhibits their binding of anti-glycoprotein E and anti-gC monoclonal antibodies.	bind
24561	8	7737	6	NULL	NULL	0	NULL	HSV-2	NULL		bind	NULL				anti-gC monoclonal antibody	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1482_1_327_s_136	11058773	3-Hydroxyphthaloyl  lg binds to HSV-1, HSV-2 and HCMV virus particles and inhibits their binding of anti-glycoprotein E and anti-gC monoclonal antibodies.	bind
24562	9	7737	6	NULL	NULL	0	NULL	HCMV	NULL		bind	NULL				anti-gC monoclonal antibody	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1482_1_327_s_136	11058773	3-Hydroxyphthaloyl  lg binds to HSV-1, HSV-2 and HCMV virus particles and inhibits their binding of anti-glycoprotein E and anti-gC monoclonal antibodies.	bind
24563	10	7737	6	NULL	NULL	0	NULL	statement 1	NULL		inhibits	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1482_1_327_s_136	11058773	3-Hydroxyphthaloyl  lg binds to HSV-1, HSV-2 and HCMV virus particles and inhibits their binding of anti-glycoprotein E and anti-gC monoclonal antibodies.	bind
24564	11	7737	6	NULL	NULL	0	NULL	statement 1	NULL		inhibits	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1482_1_327_s_136	11058773	3-Hydroxyphthaloyl  lg binds to HSV-1, HSV-2 and HCMV virus particles and inhibits their binding of anti-glycoprotein E and anti-gC monoclonal antibodies.	bind
24565	12	7737	6	NULL	NULL	0	NULL	statement 2	NULL		inhibits	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1482_1_327_s_136	11058773	3-Hydroxyphthaloyl  lg binds to HSV-1, HSV-2 and HCMV virus particles and inhibits their binding of anti-glycoprotein E and anti-gC monoclonal antibodies.	bind
24566	13	7737	6	NULL	NULL	0	NULL	statement 2	NULL		inhibits	NULL				statement 8	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1482_1_327_s_136	11058773	3-Hydroxyphthaloyl  lg binds to HSV-1, HSV-2 and HCMV virus particles and inhibits their binding of anti-glycoprotein E and anti-gC monoclonal antibodies.	bind
24567	14	7737	6	NULL	NULL	0	NULL	statement 3	NULL		inhibits	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1482_1_327_s_136	11058773	3-Hydroxyphthaloyl  lg binds to HSV-1, HSV-2 and HCMV virus particles and inhibits their binding of anti-glycoprotein E and anti-gC monoclonal antibodies.	bind
24568	15	7737	6	NULL	NULL	0	NULL	statement 3	NULL		inhibits	NULL				statement 9	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1482_1_327_s_136	11058773	3-Hydroxyphthaloyl  lg binds to HSV-1, HSV-2 and HCMV virus particles and inhibits their binding of anti-glycoprotein E and anti-gC monoclonal antibodies.	bind
31618	1	7738	5	13	NULL	NULL	NULL	p53	GP		bind					AhR	GP			mdr1 promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_7_4819_s_8	11096091	3-MC treatment of the cells increased the levels of p53 and induced p53 binding to the  mdr1 promoter in an AhR.	bind
31619	2	7738	5	13	NULL	NULL	NULL	MC	Chemical	treatment	increases					p53	GP	levels of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_7_4819_s_8	11096091	3-MC treatment of the cells increased the levels of p53 and induced p53 binding to the  mdr1 promoter in an AhR.	bind
31620	3	7738	5	13	NULL	NULL	NULL	statement 2	Process		induces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_7_4819_s_8	11096091	3-MC treatment of the cells increased the levels of p53 and induced p53 binding to the  mdr1 promoter in an AhR.	bind
24241	1	7738	6	10	NULL	0	NULL	p53	NULL		bind	NULL				AhR	NULL			mdr1 promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_7_4819_s_8	11096091	3-MC treatment of the cells increased the levels of p53 and induced p53 binding to the  mdr1 promoter in an AhR.	bind
24242	2	7738	6	NULL	NULL	0	NULL	MC	NULL	treatment with	increased	NULL				p53	NULL	levels of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_7_4819_s_8	11096091	3-MC treatment of the cells increased the levels of p53 and induced p53 binding to the  mdr1 promoter in an AhR.	bind
24348	3	7738	6	10	NULL	0	NULL	statement 2			induce					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_7_4819_s_8	11096091	3-MC treatment of the cells increased the levels of p53 and induced p53 binding to the  mdr1 promoter in an AhR.	bind
31621	1	7739	5	13	NULL	NULL	NULL	3-Methyl- cis,cis-muconate	Chemical		bind		high affinity			muconate cycloisomerase	GP	P. putida			NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_64_9_3290_s_229	9726873	3-Methyl- cis,cis-muconate binds to the  P. putida muconate cycloisomerase with a very high affinity and is converted with a moderate  kcat (Table  3), suggesting that steric problems should be of limited importance.	bind
24349	1	7739	6	NULL	NULL	0	NULL	3-Methyl- cis,cis-muconate	NULL		bind	NULL	high affinity			muconate cycloisomerase	NULL	P. putida			NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_64_9_3290_s_229	9726873	3-Methyl- cis,cis-muconate binds to the  P. putida muconate cycloisomerase with a very high affinity and is converted with a moderate  kcat (Table  3), suggesting that steric problems should be of limited importance.	bind
31629	1	7740	5	13	NULL	NULL	NULL	3-OxoC66HSL	Chemical		bind					LuxR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_6_1617_s_18	11872713	3-OxoC66HSL then binds to the transcriptional activator LuxR, and the resulting LuxR/3-oxo-C6-HSL complex triggers transcription of the luminescence ( lux) operon, resulting in the emission of light ( 39).	bind
31630	2	7740	5	13	NULL	NULL	NULL	statement 1	Process		forms					LuxR/3-oxo-C6-HSL complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_6_1617_s_18	11872713	3-OxoC66HSL then binds to the transcriptional activator LuxR, and the resulting LuxR/3-oxo-C6-HSL complex triggers transcription of the luminescence ( lux) operon, resulting in the emission of light ( 39).	bind
31631	3	7740	5	13	NULL	NULL	NULL	LuxR	GP		is a type of					transcriptional activator	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_6_1617_s_18	11872713	3-OxoC66HSL then binds to the transcriptional activator LuxR, and the resulting LuxR/3-oxo-C6-HSL complex triggers transcription of the luminescence ( lux) operon, resulting in the emission of light ( 39).	bind
31632	4	7740	5	13	NULL	NULL	NULL	LuxR/3-oxo-C6-HSL complex	GP		triggers							transcription of		 lux operon	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_6_1617_s_18	11872713	3-OxoC66HSL then binds to the transcriptional activator LuxR, and the resulting LuxR/3-oxo-C6-HSL complex triggers transcription of the luminescence ( lux) operon, resulting in the emission of light ( 39).	bind
31633	5	7740	5	13	NULL	NULL	NULL	statement 4	Process		results in					light		emission of			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_6_1617_s_18	11872713	3-OxoC66HSL then binds to the transcriptional activator LuxR, and the resulting LuxR/3-oxo-C6-HSL complex triggers transcription of the luminescence ( lux) operon, resulting in the emission of light ( 39).	bind
46778	6	7740	5	13	NULL	NULL	NULL	lux operon	NucleicAcid		is 					luminescence operon	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_6_1617_s_18	11872713	3-OxoC66HSL then binds to the transcriptional activator LuxR, and the resulting LuxR/3-oxo-C6-HSL complex triggers transcription of the luminescence ( lux) operon, resulting in the emission of light ( 39).	bind
24350	1	7740	6	10	NULL	0	NULL	3-OxoC66HSL	NULL		bind	NULL				LuxR 	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_6_1617_s_18	11872713	3-OxoC66HSL then binds to the transcriptional activator LuxR, and the resulting LuxR/3-oxo-C6-HSL complex triggers transcription of the luminescence ( lux) operon, resulting in the emission of light ( 39).	bind
24351	2	7740	6	NULL	NULL	0	NULL	statement 1	NULL		forms 	NULL				LuxR/3-oxo-C6-HSL complex 	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_6_1617_s_18	11872713	3-OxoC66HSL then binds to the transcriptional activator LuxR, and the resulting LuxR/3-oxo-C6-HSL complex triggers transcription of the luminescence ( lux) operon, resulting in the emission of light ( 39).	bind
46779	3	7740	6	10	NULL	0	NULL	LuxR	NULL		is a type of	NULL				transcriptional activator	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_6_1617_s_18	11872713	3-OxoC66HSL then binds to the transcriptional activator LuxR, and the resulting LuxR/3-oxo-C6-HSL complex triggers transcription of the luminescence ( lux) operon, resulting in the emission of light ( 39).	bind
46780	4	7740	6	10	NULL	0	NULL	LuxR/3-oxo-C6-HSL complex	NULL		triggers	NULL					NULL	transcription of		lux operon	NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_6_1617_s_18	11872713	3-OxoC66HSL then binds to the transcriptional activator LuxR, and the resulting LuxR/3-oxo-C6-HSL complex triggers transcription of the luminescence ( lux) operon, resulting in the emission of light ( 39).	bind
46781	5	7740	6	10	NULL	0	NULL	statement 4	NULL		results in	NULL				emission of light	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_6_1617_s_18	11872713	3-OxoC66HSL then binds to the transcriptional activator LuxR, and the resulting LuxR/3-oxo-C6-HSL complex triggers transcription of the luminescence ( lux) operon, resulting in the emission of light ( 39).	bind
46782	6	7740	6	10	NULL	0	NULL	lux operon	NULL		is	NULL				luminescence operon	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_6_1617_s_18	11872713	3-OxoC66HSL then binds to the transcriptional activator LuxR, and the resulting LuxR/3-oxo-C6-HSL complex triggers transcription of the luminescence ( lux) operon, resulting in the emission of light ( 39).	bind
31634	1	7741	5	13	NULL	NULL	NULL	3-oxoC88HSL	Chemical		bind		tightly			TraR	GP	active			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_19_5212_s_66	11013223	3-oxoC88HSL is bound very tightly to the active form of TraR; in previous studies prolonged dialysis was required to remove the ligand ( Zhu and Winans, 1999).	bind
24352	1	7741	6	NULL	NULL	0	NULL	3-oxoC88HSL	NULL		bind	NULL	very tightly			TraR	NULL	active form of			NULL		0	NULL	NULL	NULL	gw60_embo_19_19_5212_s_66	11013223	3-oxoC88HSL is bound very tightly to the active form of TraR; in previous studies prolonged dialysis was required to remove the ligand ( Zhu and Winans, 1999).	bind
31635	1	7742	5	13	NULL	NULL	NULL	PDK1	GP		is					3-Phosphoinositide-dependent protein kinase 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_2_253_s_5	11057898	3-Phosphoinositide-dependent protein kinase 1 (PDK1) phosphorylates and activates the p70 S6 kinase  in vivo and  in vitro.	bind
31636	2	7742	5	13	NULL	NULL	NULL	PDK1	GP		phosphorylates					p70 S6 kinase	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_cell_103_2_253_s_5	11057898	3-Phosphoinositide-dependent protein kinase 1 (PDK1) phosphorylates and activates the p70 S6 kinase  in vivo and  in vitro.	bind
31637	3	7742	5	13	NULL	NULL	NULL	statement 2	Process		activates					p70 S6 kinase	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_cell_103_2_253_s_5	11057898	3-Phosphoinositide-dependent protein kinase 1 (PDK1) phosphorylates and activates the p70 S6 kinase  in vivo and  in vitro.	bind
31638	4	7742	5	13	NULL	NULL	NULL	PDK1	GP		phosphorylates					p70 S6 kinase	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_cell_103_2_253_s_5	11057898	3-Phosphoinositide-dependent protein kinase 1 (PDK1) phosphorylates and activates the p70 S6 kinase  in vivo and  in vitro.	bind
31639	5	7742	5	13	NULL	NULL	NULL	statement 4	Process		activates					p70 S6 kinase	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_cell_103_2_253_s_5	11057898	3-Phosphoinositide-dependent protein kinase 1 (PDK1) phosphorylates and activates the p70 S6 kinase  in vivo and  in vitro.	bind
24353	1	7742	6	NULL	NULL	0	NULL	PDK1	NULL		is	NULL				Phosphoinositide-dependent protein kinase 1	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_103_2_253_s_5	11057898	3-Phosphoinositide-dependent protein kinase 1 (PDK1) phosphorylates and activates the p70 S6 kinase  in vivo and  in vitro.	bind
24354	2	7742	6	NULL	NULL	0	NULL	PDK1	NULL		phosphorylates	NULL				p70 S6 kinase	NULL				NULL	in vivo	0	NULL	NULL	NULL	gw60_cell_103_2_253_s_5	11057898	3-Phosphoinositide-dependent protein kinase 1 (PDK1) phosphorylates and activates the p70 S6 kinase  in vivo and  in vitro.	bind
24355	3	7742	6	10	NULL	0	NULL	statement 2			activates					p70 S6 kinase					NULL	in vivo	NULL	NULL	NULL	NULL	gw60_cell_103_2_253_s_5	11057898	3-Phosphoinositide-dependent protein kinase 1 (PDK1) phosphorylates and activates the p70 S6 kinase  in vivo and  in vitro.	bind
46783	4	7742	6	10	NULL	0	NULL	PDK1	NULL		phosphorylates	NULL				p70 S6 kinase	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_cell_103_2_253_s_5	11057898	3-Phosphoinositide-dependent protein kinase 1 (PDK1) phosphorylates and activates the p70 S6 kinase  in vivo and  in vitro.	bind
46784	5	7742	6	10	NULL	0	NULL	statement 4			activates					p70 S6 kinase					NULL	in vitro	NULL	NULL	NULL	NULL	gw60_cell_103_2_253_s_5	11057898	3-Phosphoinositide-dependent protein kinase 1 (PDK1) phosphorylates and activates the p70 S6 kinase  in vivo and  in vitro.	bind
31640	1	7745	5	13	NULL	NULL	NULL	DNA ligase IV	GP		bind			motif located between BRCT domains		XRCC4	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1653_s_323	11292837	30       Grawunder,U., Zimmer,D. and Lieber,M.R. (1998) DNA ligase IV binds to XRCC4 via a motif located between rather than within its BRCT domains.	bind
24356	1	7745	6	NULL	NULL	0	NULL	DNA ligase IV	NULL		bind	NULL		motif located between BRCT domains		XRCC4	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1653_s_323	11292837	30       Grawunder,U., Zimmer,D. and Lieber,M.R. (1998) DNA ligase IV binds to XRCC4 via a motif located between rather than within its BRCT domains.	bind
31641	1	7746	5	13	NULL	NULL	NULL	hnRNP L	GP		bind									cis-acting RNA sequence element	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_3_823_s_306	11809897	30       Liu,X. and Mertz,J.E. (1995) hnRNP L binds a  cis-acting RNA sequence element that enables intron-independent gene expression.	bind
31642	3	7746	5	13	NULL	NULL	NULL				enables				cis-acting RNA sequence element	statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_3_823_s_306	11809897	30       Liu,X. and Mertz,J.E. (1995) hnRNP L binds a  cis-acting RNA sequence element that enables intron-independent gene expression.	bind
46785	2	7746	5	13	NULL	NULL	NULL	gene expression	Process		is independent of					intron	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_3_823_s_306	11809897	30       Liu,X. and Mertz,J.E. (1995) hnRNP L binds a  cis-acting RNA sequence element that enables intron-independent gene expression.	bind
24357	1	7746	6	10	NULL	0	NULL	hnRNP L	NULL		bind	NULL					NULL			cis-acting RNA sequence element	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_3_823_s_306	11809897	30       Liu,X. and Mertz,J.E. (1995) hnRNP L binds a  cis-acting RNA sequence element that enables intron-independent gene expression.	bind
24358	3	7746	6	10	NULL	0	NULL		NULL		enables	NULL			cis-acting RNA sequence element	statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_3_823_s_306	11809897	30       Liu,X. and Mertz,J.E. (1995) hnRNP L binds a  cis-acting RNA sequence element that enables intron-independent gene expression.	bind
46786	2	7746	6	10	NULL	0	NULL	gene expression	NULL		is independent of	NULL				intron	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_3_823_s_306	11809897	30       Liu,X. and Mertz,J.E. (1995) hnRNP L binds a  cis-acting RNA sequence element that enables intron-independent gene expression.	bind
31643	1	7747	5	13	NULL	NULL	NULL	transcription factor	GP		bind					HER2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_23_4873_s_268	11726697	30       Noonberg,S.B., Scott,G.K., Hunt,C.A., Hogan,M.E. and Benz,C.C. (1994) Inhibition of transcription factor binding to the HER2 promoter by triplex-forming oligodeoxyribonucleotides.	bind
31644	3	7747	5	13	NULL	NULL	NULL	statement 2	Process		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_23_4873_s_268	11726697	30       Noonberg,S.B., Scott,G.K., Hunt,C.A., Hogan,M.E. and Benz,C.C. (1994) Inhibition of transcription factor binding to the HER2 promoter by triplex-forming oligodeoxyribonucleotides.	bind
46787	2	7747	5	13	NULL	NULL	NULL	oligodeoxyribonucleotides	NucleicAcid		forms					triplex	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_23_4873_s_268	11726697	30       Noonberg,S.B., Scott,G.K., Hunt,C.A., Hogan,M.E. and Benz,C.C. (1994) Inhibition of transcription factor binding to the HER2 promoter by triplex-forming oligodeoxyribonucleotides.	bind
24359	1	7747	6	NULL	NULL	0	NULL	transcription factor	NULL		bind	NULL				HER2	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_23_4873_s_268	11726697	30       Noonberg,S.B., Scott,G.K., Hunt,C.A., Hogan,M.E. and Benz,C.C. (1994) Inhibition of transcription factor binding to the HER2 promoter by triplex-forming oligodeoxyribonucleotides.	bind
24360	3	7747	6	10	NULL	0	NULL	statement 2	NULL		inhibits	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_23_4873_s_268	11726697	30       Noonberg,S.B., Scott,G.K., Hunt,C.A., Hogan,M.E. and Benz,C.C. (1994) Inhibition of transcription factor binding to the HER2 promoter by triplex-forming oligodeoxyribonucleotides.	bind
46788	2	7747	6	10	NULL	0	NULL	oligodeoxyribonucleotides	NULL		forms	NULL				triplex	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_23_4873_s_268	11726697	30       Noonberg,S.B., Scott,G.K., Hunt,C.A., Hogan,M.E. and Benz,C.C. (1994) Inhibition of transcription factor binding to the HER2 promoter by triplex-forming oligodeoxyribonucleotides.	bind
31645	1	7748	5	13	NULL	NULL	NULL	Vav	GP		bind					hnRNP	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_6_1300_s_348	11238996	30       Romero,F., Germani,A., Puvion,E., Camonis,J., Varin-Blank,N., Gisselbrecht,S. and Fischer,S. (1998) Vav binding to heterogeneous nuclear ribonucleoprotein (hnRNP) C. Evidence for Vav-hnRNP interactions in an RNA-dependent manner.	bind
31654	2	7748	5	13	NULL	NULL	NULL	hnRNP	GP		is					heterogeneous nuclear ribonucleoprotein	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_6_1300_s_348	11238996	30       Romero,F., Germani,A., Puvion,E., Camonis,J., Varin-Blank,N., Gisselbrecht,S. and Fischer,S. (1998) Vav binding to heterogeneous nuclear ribonucleoprotein (hnRNP) C. Evidence for Vav-hnRNP interactions in an RNA-dependent manner.	bind
31656	3	7748	5	13	NULL	NULL	NULL	statement 1	Process		is dependent on					RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_6_1300_s_348	11238996	30       Romero,F., Germani,A., Puvion,E., Camonis,J., Varin-Blank,N., Gisselbrecht,S. and Fischer,S. (1998) Vav binding to heterogeneous nuclear ribonucleoprotein (hnRNP) C. Evidence for Vav-hnRNP interactions in an RNA-dependent manner.	bind
24361	1	7748	6	NULL	NULL	0	NULL	Vav	NULL		bind	NULL				hnRNP	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_6_1300_s_348	11238996	30       Romero,F., Germani,A., Puvion,E., Camonis,J., Varin-Blank,N., Gisselbrecht,S. and Fischer,S. (1998) Vav binding to heterogeneous nuclear ribonucleoprotein (hnRNP) C. Evidence for Vav-hnRNP interactions in an RNA-dependent manner.	bind
24362	2	7748	6	NULL	NULL	0	NULL	hnRNP	NULL		is	NULL				heterogeneous nuclear ribonucleoprotein	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_6_1300_s_348	11238996	30       Romero,F., Germani,A., Puvion,E., Camonis,J., Varin-Blank,N., Gisselbrecht,S. and Fischer,S. (1998) Vav binding to heterogeneous nuclear ribonucleoprotein (hnRNP) C. Evidence for Vav-hnRNP interactions in an RNA-dependent manner.	bind
24363	3	7748	6	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				RNA	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_6_1300_s_348	11238996	30       Romero,F., Germani,A., Puvion,E., Camonis,J., Varin-Blank,N., Gisselbrecht,S. and Fischer,S. (1998) Vav binding to heterogeneous nuclear ribonucleoprotein (hnRNP) C. Evidence for Vav-hnRNP interactions in an RNA-dependent manner.	bind
31658	1	7749	5	13	NULL	NULL	NULL	nucleosomal DNA	NucleicAcid		regulates					hat1 acetyltransferase	GP	human	core-histone binding subunit		NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_629_s_333	11160883	30       Verreault,A., Kaufman,P.D., Kobayashi,R. and Stillman,B. (1998) Nucleosomal DNA regulates the core-histone binding subunit of the human hat1 acetyltransferase.	bind
24364	1	7749	6	NULL	NULL	0	NULL	Nucleosomal DNA	NULL		regulates	NULL				Hat1 acetyltransferase	NULL	human	core-histone binding subunit		NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_629_s_333	11160883	30       Verreault,A., Kaufman,P.D., Kobayashi,R. and Stillman,B. (1998) Nucleosomal DNA regulates the core-histone binding subunit of the human hat1 acetyltransferase.	bind
31659	1	7750	5	13	NULL	NULL	NULL	FGF-1	GP		bind					FGFR-2 IIIb	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_3_207_s_218	10926871	30  Both FGF-1 and FGF-7 can bind to FGFR-2 IIIb. 31  It is tempting to speculate that different members of the FGF gene family exert similar biological functions, with regard to the regulation of the branching morphogenesis of different embryonic structures.	bind
31660	2	7750	5	13	NULL	NULL	NULL	FGF-7	GP		bind					FGFR-2 IIIb	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_3_207_s_218	10926871	30  Both FGF-1 and FGF-7 can bind to FGFR-2 IIIb. 31  It is tempting to speculate that different members of the FGF gene family exert similar biological functions, with regard to the regulation of the branching morphogenesis of different embryonic structures.	bind
46789	3	7750	5	13	NULL	NULL	NULL	FGF gene family members	GP		play a role in					branching morphogenesis of different embryonic structures	Process	regulation of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_3_207_s_218	10926871	30  Both FGF-1 and FGF-7 can bind to FGFR-2 IIIb. 31  It is tempting to speculate that different members of the FGF gene family exert similar biological functions, with regard to the regulation of the branching morphogenesis of different embryonic structures.	bind
24365	1	7750	6	NULL	NULL	0	NULL	FGF-1	NULL		bind	NULL				FGFR-2 IIIb	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_3_207_s_218	10926871	30  Both FGF-1 and FGF-7 can bind to FGFR-2 IIIb. 31  It is tempting to speculate that different members of the FGF gene family exert similar biological functions, with regard to the regulation of the branching morphogenesis of different embryonic structures.	bind
24366	2	7750	6	NULL	NULL	0	NULL	FGF-7	NULL		bind	NULL				FGFR-2 IIIb	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_3_207_s_218	10926871	30  Both FGF-1 and FGF-7 can bind to FGFR-2 IIIb. 31  It is tempting to speculate that different members of the FGF gene family exert similar biological functions, with regard to the regulation of the branching morphogenesis of different embryonic structures.	bind
24367	3	7750	6	NULL	NULL	0	NULL	FGF gene family members	NULL		plays a role in	NULL				branching morphogenesis of embryonic structures	NULL	regulation of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_3_207_s_218	10926871	30  Both FGF-1 and FGF-7 can bind to FGFR-2 IIIb. 31  It is tempting to speculate that different members of the FGF gene family exert similar biological functions, with regard to the regulation of the branching morphogenesis of different embryonic structures.	bind
31662	1	7751	5	13	NULL	NULL	NULL	substance P	GP		inhibits					endothelin-1	GP	 binding of			NULL	rat cardiac membranes in vitro	NULL	NULL	NULL	NULL	gw60_circulation_102_14_1617_s_136	11015337	30  In rat cardiac membranes in vitro, specific binding of endothelin-1 can be inhibited by substance P.	bind
24368	1	7751	6	NULL	NULL	0	NULL	substance P	NULL		inhibits	NULL				endothelin-1	NULL	binding of			NULL	rat cardiac membranes in vitro	0	NULL	NULL	NULL	gw60_circulation_102_14_1617_s_136	11015337	30  In rat cardiac membranes in vitro, specific binding of endothelin-1 can be inhibited by substance P.	bind
31666	1	7752	5	13	NULL	NULL	NULL	HK	GP		bind					glycoprotein Ib/IX complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2245_s_144	10479669	30  Recently, we 31  and others 32  have shown that HK binds to the glycoprotein Ib/IX complex.	bind
24369	1	7752	6	NULL	NULL	0	NULL	HK	NULL		bind	NULL				glycoprotein Ib/IX complex	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2245_s_144	10479669	30  Recently, we 31  and others 32  have shown that HK binds to the glycoprotein Ib/IX complex.	bind
31669	1	7753	5	13	NULL	NULL	NULL	WDR1 proteins	GP	yeast	bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_5_460_s_170	11249868	30  The highly homologous yeast and slime mold WDR1 proteins bind actin, which suggests that WDR1 protein may be an actin binding protein as well.	bind
31670	2	7753	5	13	NULL	NULL	NULL	WDR1 proteins	GP	slime mold	bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_5_460_s_170	11249868	30  The highly homologous yeast and slime mold WDR1 proteins bind actin, which suggests that WDR1 protein may be an actin binding protein as well.	bind
31672	3	7753	5	13	NULL	NULL	NULL	WDR1 proteins	GP	yeast	is homologus to		highly			WDR1 proteins	GP	slime mold			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_5_460_s_170	11249868	30  The highly homologous yeast and slime mold WDR1 proteins bind actin, which suggests that WDR1 protein may be an actin binding protein as well.	bind
24370	1	7753	6	NULL	NULL	0	NULL	WDR1 protein	NULL	yeast	bind	NULL				actin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_88_5_460_s_170	11249868	30  The highly homologous yeast and slime mold WDR1 proteins bind actin, which suggests that WDR1 protein may be an actin binding protein as well.	bind
24371	2	7753	6	NULL	NULL	0	NULL	WDR1 protein	NULL	slime mold	bind	NULL				actin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_88_5_460_s_170	11249868	30  The highly homologous yeast and slime mold WDR1 proteins bind actin, which suggests that WDR1 protein may be an actin binding protein as well.	bind
46823	3	7753	6	10	NULL	0	NULL	WDR1 proteins	NULL	yeast	is homologous to	NULL				WDR1 proteins	NULL	slime mold			NULL		0	NULL	NULL	NULL	gw60_circulationres_88_5_460_s_170	11249868	30  The highly homologous yeast and slime mold WDR1 proteins bind actin, which suggests that WDR1 protein may be an actin binding protein as well.	bind
31674	1	7754	5	13	NULL	NULL	NULL	Src	GP		does not undergo					palmitylation	Process				NULL	resting rat platelets	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3278_s_202	9409323	30 - 32 The fact that Src is not palmitylated, but a portion is still Triton-insoluble in resting rat platelets, suggests that Src in resting rat platelets is not bound to the same Triton-insoluble macromolecules as the other Src family members.	bind
31683	2	7754	5	13	NULL	NULL	NULL	Src	GP		does not bind					macromolecules	CellComponent	Triton-insoluble			NULL	resting rat platelets	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3278_s_202	9409323	30 - 32 The fact that Src is not palmitylated, but a portion is still Triton-insoluble in resting rat platelets, suggests that Src in resting rat platelets is not bound to the same Triton-insoluble macromolecules as the other Src family members.	bind
24372	1	7754	6	NULL	NULL	0	NULL	Src	NULL		does not bind	NULL				macromolecules	NULL	triton-insoluble			NULL	resting rat platelets	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3278_s_202	9409323	30 - 32 The fact that Src is not palmitylated, but a portion is still Triton-insoluble in resting rat platelets, suggests that Src in resting rat platelets is not bound to the same Triton-insoluble macromolecules as the other Src family members.	bind
24373	2	7754	6	10	NULL	0	NULL	src			does not undergo					palmitylation					NULL	resting rat platelets	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3278_s_202	9409323	30 - 32 The fact that Src is not palmitylated, but a portion is still Triton-insoluble in resting rat platelets, suggests that Src in resting rat platelets is not bound to the same Triton-insoluble macromolecules as the other Src family members.	bind
31684	1	7755	5	13	NULL	NULL	NULL	F1 	GP		bind					F0	GP	mutant			NULL	in membranes	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_23797_s_140	15849185	30 - 80% of the F1 ATPase activity was inhibited when F1 was bound to mutant F0 in membranes, as estimated from the increase in ATPase activity after detachment from the membranes.	bind
31685	2	7755	5	13	NULL	NULL	NULL	statement 1	Process		inhibits					F1 ATPase activity	GP				NULL	membranes	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_23797_s_140	15849185	30 - 80% of the F1 ATPase activity was inhibited when F1 was bound to mutant F0 in membranes, as estimated from the increase in ATPase activity after detachment from the membranes.	bind
24374	1	7755	6	NULL	NULL	0	NULL	F1	NULL		bind	NULL				F0	NULL	mutant			NULL	membranes	0	NULL	NULL	NULL	gw70_jbiolchem_280_25_23797_s_140	15849185	30 - 80% of the F1 ATPase activity was inhibited when F1 was bound to mutant F0 in membranes, as estimated from the increase in ATPase activity after detachment from the membranes.	bind
24375	2	7755	6	10	NULL	0	NULL	statement 1			inhibits					F1 ATPase activity					NULL	membranes	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_23797_s_140	15849185	30 - 80% of the F1 ATPase activity was inhibited when F1 was bound to mutant F0 in membranes, as estimated from the increase in ATPase activity after detachment from the membranes.	bind
31686	1	7757	5	13	NULL	NULL	NULL	NHE-1	GP		bind		strongly	cytoplasmic domain		calmodulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_8_824_s_228	9776729	30 31 32  Binding experiments with calmodulin-Sepharose, as well as fluorescence measurements with dansylated calmodulin, revealed that the NHE-1 cytoplasmic domain strongly binds calmodulin in a Ca2+-dependent manner.	bind
31687	2	7757	5	13	NULL	NULL	NULL	statement 1	Process		is dependent on					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_8_824_s_228	9776729	30 31 32  Binding experiments with calmodulin-Sepharose, as well as fluorescence measurements with dansylated calmodulin, revealed that the NHE-1 cytoplasmic domain strongly binds calmodulin in a Ca2+-dependent manner.	bind
24376	1	7757	6	NULL	NULL	0	NULL	NHE-1	NULL		bind	NULL	strongly	cytoplasmic domain		calmodulin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_8_824_s_228	9776729	30 31 32  Binding experiments with calmodulin-Sepharose, as well as fluorescence measurements with dansylated calmodulin, revealed that the NHE-1 cytoplasmic domain strongly binds calmodulin in a Ca2+-dependent manner.	bind
24377	2	7757	6	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				Ca2+	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_8_824_s_228	9776729	30 31 32  Binding experiments with calmodulin-Sepharose, as well as fluorescence measurements with dansylated calmodulin, revealed that the NHE-1 cytoplasmic domain strongly binds calmodulin in a Ca2+-dependent manner.	bind
31690	1	7758	5	13	NULL	NULL	NULL	tie-2	GP		contains					tie-2	GP			GATA consensus sequences in promoter	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_7_749_s_197	12637368	30 Although no direct proof for a direct interaction between GATA-4 and Ets-1 or Ets-2 is available, the notion that several genes involved in vascular biology have both GATA and Ets consensus sequences in their promoters (eg, in the tie-2 31 and Flk-1 32 genes) and proven cooperative binding between Ets-1 and Ets-2 with GATA-3 33 may give further clues for the mode of action by which Ets transcription factors influence coronary development.	bind
31691	2	7758	5	13	NULL	NULL	NULL	tie-2	GP		contains					tie-2	GP			Ets consensus sequences in promoter	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_7_749_s_197	12637368	30 Although no direct proof for a direct interaction between GATA-4 and Ets-1 or Ets-2 is available, the notion that several genes involved in vascular biology have both GATA and Ets consensus sequences in their promoters (eg, in the tie-2 31 and Flk-1 32 genes) and proven cooperative binding between Ets-1 and Ets-2 with GATA-3 33 may give further clues for the mode of action by which Ets transcription factors influence coronary development.	bind
31692	3	7758	5	13	NULL	NULL	NULL	Flk-1	GP		contains					Flk-1	GP			GATA consensus sequences in promoter	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_7_749_s_197	12637368	30 Although no direct proof for a direct interaction between GATA-4 and Ets-1 or Ets-2 is available, the notion that several genes involved in vascular biology have both GATA and Ets consensus sequences in their promoters (eg, in the tie-2 31 and Flk-1 32 genes) and proven cooperative binding between Ets-1 and Ets-2 with GATA-3 33 may give further clues for the mode of action by which Ets transcription factors influence coronary development.	bind
31693	4	7758	5	13	NULL	NULL	NULL	Flk-1	GP		contains					Flk-1	GP			Ets consensus sequences in promoter	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_7_749_s_197	12637368	30 Although no direct proof for a direct interaction between GATA-4 and Ets-1 or Ets-2 is available, the notion that several genes involved in vascular biology have both GATA and Ets consensus sequences in their promoters (eg, in the tie-2 31 and Flk-1 32 genes) and proven cooperative binding between Ets-1 and Ets-2 with GATA-3 33 may give further clues for the mode of action by which Ets transcription factors influence coronary development.	bind
31694	5	7758	5	13	NULL	NULL	NULL	Ets-1	GP		bind					GATA-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_7_749_s_197	12637368	30 Although no direct proof for a direct interaction between GATA-4 and Ets-1 or Ets-2 is available, the notion that several genes involved in vascular biology have both GATA and Ets consensus sequences in their promoters (eg, in the tie-2 31 and Flk-1 32 genes) and proven cooperative binding between Ets-1 and Ets-2 with GATA-3 33 may give further clues for the mode of action by which Ets transcription factors influence coronary development.	bind
31695	6	7758	5	13	NULL	NULL	NULL	Ets-2	GP		bind					GATA-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_7_749_s_197	12637368	30 Although no direct proof for a direct interaction between GATA-4 and Ets-1 or Ets-2 is available, the notion that several genes involved in vascular biology have both GATA and Ets consensus sequences in their promoters (eg, in the tie-2 31 and Flk-1 32 genes) and proven cooperative binding between Ets-1 and Ets-2 with GATA-3 33 may give further clues for the mode of action by which Ets transcription factors influence coronary development.	bind
31696	7	7758	5	13	NULL	NULL	NULL	statement 5	Process		cooperative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_7_749_s_197	12637368	30 Although no direct proof for a direct interaction between GATA-4 and Ets-1 or Ets-2 is available, the notion that several genes involved in vascular biology have both GATA and Ets consensus sequences in their promoters (eg, in the tie-2 31 and Flk-1 32 genes) and proven cooperative binding between Ets-1 and Ets-2 with GATA-3 33 may give further clues for the mode of action by which Ets transcription factors influence coronary development.	bind
31697	8	7758	5	13	NULL	NULL	NULL	Ets transcription factors	GP		influence					coronary development	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_7_749_s_197	12637368	30 Although no direct proof for a direct interaction between GATA-4 and Ets-1 or Ets-2 is available, the notion that several genes involved in vascular biology have both GATA and Ets consensus sequences in their promoters (eg, in the tie-2 31 and Flk-1 32 genes) and proven cooperative binding between Ets-1 and Ets-2 with GATA-3 33 may give further clues for the mode of action by which Ets transcription factors influence coronary development.	bind
24378	1	7758	6	NULL	NULL	0	NULL	Ets-1	NULL		bind	NULL				GATA-3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_92_7_749_s_197	12637368	30 Although no direct proof for a direct interaction between GATA-4 and Ets-1 or Ets-2 is available, the notion that several genes involved in vascular biology have both GATA and Ets consensus sequences in their promoters (eg, in the tie-2 31 and Flk-1 32 genes) and proven cooperative binding between Ets-1 and Ets-2 with GATA-3 33 may give further clues for the mode of action by which Ets transcription factors influence coronary development.	bind
24379	2	7758	6	NULL	NULL	0	NULL	Ets-2	NULL		bind	NULL				GATA-3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_92_7_749_s_197	12637368	30 Although no direct proof for a direct interaction between GATA-4 and Ets-1 or Ets-2 is available, the notion that several genes involved in vascular biology have both GATA and Ets consensus sequences in their promoters (eg, in the tie-2 31 and Flk-1 32 genes) and proven cooperative binding between Ets-1 and Ets-2 with GATA-3 33 may give further clues for the mode of action by which Ets transcription factors influence coronary development.	bind
24380	3	7758	6	NULL	NULL	0	NULL	statement 1	NULL		acts in cooperation with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_92_7_749_s_197	12637368	30 Although no direct proof for a direct interaction between GATA-4 and Ets-1 or Ets-2 is available, the notion that several genes involved in vascular biology have both GATA and Ets consensus sequences in their promoters (eg, in the tie-2 31 and Flk-1 32 genes) and proven cooperative binding between Ets-1 and Ets-2 with GATA-3 33 may give further clues for the mode of action by which Ets transcription factors influence coronary development.	bind
24381	4	7758	6	NULL	NULL	0	NULL	Ets transcription factors	NULL		influence	NULL				coronary development	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_92_7_749_s_197	12637368	30 Although no direct proof for a direct interaction between GATA-4 and Ets-1 or Ets-2 is available, the notion that several genes involved in vascular biology have both GATA and Ets consensus sequences in their promoters (eg, in the tie-2 31 and Flk-1 32 genes) and proven cooperative binding between Ets-1 and Ets-2 with GATA-3 33 may give further clues for the mode of action by which Ets transcription factors influence coronary development.	bind
31698	1	7759	5	13	NULL	NULL	NULL	PTX3	GP		bind					fibroblast growth factor-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_16_2349_s_103	15477419	30 Finally, recent results indicate that PTX3 binds and inactivates fibroblast growth factor-2.	bind
31699	2	7759	5	13	NULL	NULL	NULL	statement 1	Process		inactivates					fibroblast growth factor-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_16_2349_s_103	15477419	30 Finally, recent results indicate that PTX3 binds and inactivates fibroblast growth factor-2.	bind
24382	1	7759	6	NULL	NULL	0	NULL	PTX3	NULL		bind	NULL				fibroblast growth factor-2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_110_16_2349_s_103	15477419	30 Finally, recent results indicate that PTX3 binds and inactivates fibroblast growth factor-2.	bind
24383	2	7759	6	10	NULL	0	NULL	statement 1			inactivates					fibroblast growth factor-2					NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_16_2349_s_103	15477419	30 Finally, recent results indicate that PTX3 binds and inactivates fibroblast growth factor-2.	bind
31700	1	7760	5	13	NULL	NULL	NULL	p65	GP		bind					DNA	NucleicAcid				NULL	LPS-treated cells	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1213_s_91	15718493	30 However, no p65-DNA binding was observed in the nuclear extracts of the cells treated with mmLDL, whereas the LPS-treated cells showed the expected p65-DNA binding ( Figure 1B).	bind
31701	2	7760	5	13	NULL	NULL	NULL	p65	GP		does not bind					DNA	NucleicAcid				NULL	nuclear extracts of cells treated with mmLDL	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1213_s_91	15718493	30 However, no p65-DNA binding was observed in the nuclear extracts of the cells treated with mmLDL, whereas the LPS-treated cells showed the expected p65-DNA binding ( Figure 1B).	bind
24384	1	7760	6	NULL	NULL	0	NULL	p65	NULL		does not bind	NULL				DNA	NULL				NULL	nuclear extracts of the cells treated with mmLDL	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1213_s_91	15718493	30 However, no p65-DNA binding was observed in the nuclear extracts of the cells treated with mmLDL, whereas the LPS-treated cells showed the expected p65-DNA binding ( Figure 1B).	bind
24385	2	7760	6	NULL	NULL	0	NULL	p65	NULL		bind	NULL				DNA	NULL				NULL	nuclear extracts of the cells treated with LPS	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1213_s_91	15718493	30 However, no p65-DNA binding was observed in the nuclear extracts of the cells treated with mmLDL, whereas the LPS-treated cells showed the expected p65-DNA binding ( Figure 1B).	bind
31702	1	7761	5	13	NULL	NULL	NULL	NO	Chemical		supress		may			PKG	GP	expression of			NULL	VSMCs	NULL	NULL	NULL	NULL	gw60_circulationres_90_4_405_s_220	11884369	30 In VSMCs, NO may suppress PKG expression by directly inhibiting Sp1 transcription factor binding activity to the PKG promoter, an observation supported by the direct effect of NO on Sp1 binding in nuclear extracts of cells pretreated with NO donors.	bind
31703	2	7761	5	13	NULL	NULL	NULL	Sp1	GP		bind					PKG	GP			promoter	NULL	VSMCs	NULL	NULL	NULL	NULL	gw60_circulationres_90_4_405_s_220	11884369	30 In VSMCs, NO may suppress PKG expression by directly inhibiting Sp1 transcription factor binding activity to the PKG promoter, an observation supported by the direct effect of NO on Sp1 binding in nuclear extracts of cells pretreated with NO donors.	bind
31704	3	7761	5	13	NULL	NULL	NULL	Sp1	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_4_405_s_220	11884369	30 In VSMCs, NO may suppress PKG expression by directly inhibiting Sp1 transcription factor binding activity to the PKG promoter, an observation supported by the direct effect of NO on Sp1 binding in nuclear extracts of cells pretreated with NO donors.	bind
31705	4	7761	5	NULL	NULL	NULL	NULL	NO	Chemical		inhibits		directly			statement 1	Process				NULL	VSMCs	NULL	NULL	NULL	NULL	gw60_circulationres_90_4_405_s_220	11884369	30 In VSMCs, NO may suppress PKG expression by directly inhibiting Sp1 transcription factor binding activity to the PKG promoter, an observation supported by the direct effect of NO on Sp1 binding in nuclear extracts of cells pretreated with NO donors.	bind
31706	5	7761	5	NULL	NULL	NULL	NULL	statement 4	Process		leads to					statement 1	Process				NULL	VSMCs	NULL	NULL	NULL	NULL	gw60_circulationres_90_4_405_s_220	11884369	30 In VSMCs, NO may suppress PKG expression by directly inhibiting Sp1 transcription factor binding activity to the PKG promoter, an observation supported by the direct effect of NO on Sp1 binding in nuclear extracts of cells pretreated with NO donors.	bind
31707	6	7761	5	13	NULL	NULL	NULL	NO	Chemical		effects		directly			Sp1	GP	binding of			NULL	in nuclear extracts of cells pretreated with NO donors	NULL	NULL	NULL	NULL	gw60_circulationres_90_4_405_s_220	11884369	30 In VSMCs, NO may suppress PKG expression by directly inhibiting Sp1 transcription factor binding activity to the PKG promoter, an observation supported by the direct effect of NO on Sp1 binding in nuclear extracts of cells pretreated with NO donors.	bind
68025	1	7761	5	11	NULL	0	NULL	 NO	Chemical		suppress		may			PKG	GP	expression			NULL	In VSMCs	0	NULL	NULL	NULL	gw60_circulationres_90_4_405_s_220	11884369	30 In VSMCs, NO may suppress PKG expression by directly inhibiting Sp1 transcription factor binding activity to the PKG promoter, an observation supported by the direct effect of NO on Sp1 binding in nuclear extracts of cells pretreated with NO donors.	bind
68026	1	7761	5	11	NULL	0	NULL	Sp1	GP		is					 transcription factor	GP				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_4_405_s_220	11884369	30 In VSMCs, NO may suppress PKG expression by directly inhibiting Sp1 transcription factor binding activity to the PKG promoter, an observation supported by the direct effect of NO on Sp1 binding in nuclear extracts of cells pretreated with NO donors.	bind
68027	1	7761	5	11	NULL	0	NULL	Sp1	GP		binding					 PKG	GP			promoter	NULL		0	NULL	NULL	NULL	gw60_circulationres_90_4_405_s_220	11884369	30 In VSMCs, NO may suppress PKG expression by directly inhibiting Sp1 transcription factor binding activity to the PKG promoter, an observation supported by the direct effect of NO on Sp1 binding in nuclear extracts of cells pretreated with NO donors.	bind
24386	1	7761	6	10	NULL	0	NULL	Sp1			bind					PKG				promoter	NULL	VSMC	NULL	NULL	NULL	NULL	gw60_circulationres_90_4_405_s_220	11884369	30 In VSMCs, NO may suppress PKG expression by directly inhibiting Sp1 transcription factor binding activity to the PKG promoter, an observation supported by the direct effect of NO on Sp1 binding in nuclear extracts of cells pretreated with NO donors.	bind
24387	2	7761	6	10	NULL	0	NULL	NO			effects		directly			Sp1		binding of			NULL	nuclear extracts of cells pretreated with NO donors	NULL	NULL	NULL	NULL	gw60_circulationres_90_4_405_s_220	11884369	30 In VSMCs, NO may suppress PKG expression by directly inhibiting Sp1 transcription factor binding activity to the PKG promoter, an observation supported by the direct effect of NO on Sp1 binding in nuclear extracts of cells pretreated with NO donors.	bind
24388	3	7761	6	NULL	NULL	0	NULL	NO	NULL		inhibits	NULL				statement 1	NULL				NULL	VSMC	0	NULL	NULL	NULL	gw60_circulationres_90_4_405_s_220	11884369	30 In VSMCs, NO may suppress PKG expression by directly inhibiting Sp1 transcription factor binding activity to the PKG promoter, an observation supported by the direct effect of NO on Sp1 binding in nuclear extracts of cells pretreated with NO donors.	bind
24389	4	7761	6	NULL	NULL	0	NULL	NO	NULL		suppress	NULL	may			PKG	NULL	expression of			NULL	VSMC	0	NULL	NULL	NULL	gw60_circulationres_90_4_405_s_220	11884369	30 In VSMCs, NO may suppress PKG expression by directly inhibiting Sp1 transcription factor binding activity to the PKG promoter, an observation supported by the direct effect of NO on Sp1 binding in nuclear extracts of cells pretreated with NO donors.	bind
24390	5	7761	6	NULL	NULL	0	NULL	statement 4	NULL		occurs by	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_4_405_s_220	11884369	30 In VSMCs, NO may suppress PKG expression by directly inhibiting Sp1 transcription factor binding activity to the PKG promoter, an observation supported by the direct effect of NO on Sp1 binding in nuclear extracts of cells pretreated with NO donors.	bind
46824	6	7761	6	10	NULL	0	NULL	Sp1	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_4_405_s_220	11884369	30 In VSMCs, NO may suppress PKG expression by directly inhibiting Sp1 transcription factor binding activity to the PKG promoter, an observation supported by the direct effect of NO on Sp1 binding in nuclear extracts of cells pretreated with NO donors.	bind
31708	1	7762	5	13	NULL	NULL	NULL	JNK	GP		phosphorylates					c-Jun	GP		Ser-63		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_5_970_s_185	15718494	30 JNK phosphorylates c-Jun at Ser-63, resulting in the binding of c-Jun to the CREB-binding protein/p300 family of transcriptional coactivators.	bind
31709	2	7762	5	13	NULL	NULL	NULL	c-Jun	GP		bind					CREB-binding protein/p300	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_5_970_s_185	15718494	30 JNK phosphorylates c-Jun at Ser-63, resulting in the binding of c-Jun to the CREB-binding protein/p300 family of transcriptional coactivators.	bind
31710	3	7762	5	13	NULL	NULL	NULL	statement 1	Process		results in					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_5_970_s_185	15718494	30 JNK phosphorylates c-Jun at Ser-63, resulting in the binding of c-Jun to the CREB-binding protein/p300 family of transcriptional coactivators.	bind
31711	4	7762	5	13	NULL	NULL	NULL	CREB-binding protein/p300	GP		is a family of					transcriptional coactivators	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_5_970_s_185	15718494	30 JNK phosphorylates c-Jun at Ser-63, resulting in the binding of c-Jun to the CREB-binding protein/p300 family of transcriptional coactivators.	bind
24412	1	7762	6	NULL	NULL	0	NULL	JNK	NULL		phosphorylates	NULL				c-jun	NULL		Ser-63		NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_5_970_s_185	15718494	30 JNK phosphorylates c-Jun at Ser-63, resulting in the binding of c-Jun to the CREB-binding protein/p300 family of transcriptional coactivators.	bind
24417	2	7762	6	10	NULL	0	NULL	c-Jun	NULL		bind	NULL				CREB-binding protein/p300 	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_5_970_s_185	15718494	30 JNK phosphorylates c-Jun at Ser-63, resulting in the binding of c-Jun to the CREB-binding protein/p300 family of transcriptional coactivators.	bind
24418	3	7762	6	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_5_970_s_185	15718494	30 JNK phosphorylates c-Jun at Ser-63, resulting in the binding of c-Jun to the CREB-binding protein/p300 family of transcriptional coactivators.	bind
46825	4	7762	6	10	NULL	0	NULL	CREB-binding protein/p300	NULL		is a type of	NULL				transcriptional coactivators	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_5_970_s_185	15718494	30 JNK phosphorylates c-Jun at Ser-63, resulting in the binding of c-Jun to the CREB-binding protein/p300 family of transcriptional coactivators.	bind
31765	1	7764	5	13	NULL	NULL	NULL	GTP	Chemical		bind					p3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_5_2553_s_102	9446556	30 mug of anti-p3 or anti-p5 antibodies reduced hydrolysis of GTP bound to p3 by only 26.5  plus-or-minus  2.3% and 32.3  plus-or-minus  1.9%, respectively, when added to p3 simultaneously with p5 (data not shown).	bind
31766	2	7764	5	13	NULL	NULL	NULL	anti-p3 antibodies	GP		reduces					statement 1	Process	hydrolysis of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_5_2553_s_102	9446556	30 mug of anti-p3 or anti-p5 antibodies reduced hydrolysis of GTP bound to p3 by only 26.5  plus-or-minus  2.3% and 32.3  plus-or-minus  1.9%, respectively, when added to p3 simultaneously with p5 (data not shown).	bind
31767	3	7764	5	13	NULL	NULL	NULL	anti-p5 antibodies	GP		reduces					statement 1	Process	hydrolysis of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_5_2553_s_102	9446556	30 mug of anti-p3 or anti-p5 antibodies reduced hydrolysis of GTP bound to p3 by only 26.5  plus-or-minus  2.3% and 32.3  plus-or-minus  1.9%, respectively, when added to p3 simultaneously with p5 (data not shown).	bind
24422	1	7764	6	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				p3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2553_s_102	9446556	30 mug of anti-p3 or anti-p5 antibodies reduced hydrolysis of GTP bound to p3 by only 26.5  plus-or-minus  2.3% and 32.3  plus-or-minus  1.9%, respectively, when added to p3 simultaneously with p5 (data not shown).	bind
24423	2	7764	6	10	NULL	0	NULL	anti-p3 antibodies	NULL		reduce	NULL				statement 1	NULL	hydrolysis of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_5_2553_s_102	9446556	30 mug of anti-p3 or anti-p5 antibodies reduced hydrolysis of GTP bound to p3 by only 26.5  plus-or-minus  2.3% and 32.3  plus-or-minus  1.9%, respectively, when added to p3 simultaneously with p5 (data not shown).	bind
24424	3	7764	6	10	NULL	0	NULL	anti-p5 antibodies	NULL		reduce	NULL				statement 1	NULL	 hydrolysis of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_5_2553_s_102	9446556	30 mug of anti-p3 or anti-p5 antibodies reduced hydrolysis of GTP bound to p3 by only 26.5  plus-or-minus  2.3% and 32.3  plus-or-minus  1.9%, respectively, when added to p3 simultaneously with p5 (data not shown).	bind
31712	1	7766	5	13	NULL	NULL	NULL	VBP	GP		bind									cis element	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_44_34826_s_144	10942764	30 nm VBP was bound to its cis element and competed with 1, 10, or 100 molar eq of the indicated A-ZIP.	bind
31713	2	7766	5	13	NULL	NULL	NULL	A-ZIP	GP		bind									cis element	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_44_34826_s_144	10942764	30 nm VBP was bound to its cis element and competed with 1, 10, or 100 molar eq of the indicated A-ZIP.	bind
31714	3	7766	5	13	NULL	NULL	NULL	statement 1	Process		competes with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_44_34826_s_144	10942764	30 nm VBP was bound to its cis element and competed with 1, 10, or 100 molar eq of the indicated A-ZIP.	bind
24425	1	7766	6	NULL	NULL	0	NULL	VBP	NULL		bind	NULL					NULL			cis-element	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_44_34826_s_144	10942764	30 nm VBP was bound to its cis element and competed with 1, 10, or 100 molar eq of the indicated A-ZIP.	bind
24426	2	7766	6	NULL	NULL	0	NULL	A-ZIP	NULL		bind	NULL					NULL			cis-element	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_44_34826_s_144	10942764	30 nm VBP was bound to its cis element and competed with 1, 10, or 100 molar eq of the indicated A-ZIP.	bind
24427	3	7766	6	NULL	NULL	0	NULL	statement 1	NULL		competes	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_44_34826_s_144	10942764	30 nm VBP was bound to its cis element and competed with 1, 10, or 100 molar eq of the indicated A-ZIP.	bind
31715	1	7767	5	13	NULL	NULL	NULL	IgM autoantibodies	GP		bind					MDA-LDL	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_108_9_1059_s_63	12912807	30 Plasma titers of IgM and IgG autoantibodies binding to MDA-LDL and Cu-OxLDL were determined by chemiluminescence ELISA as previously described.	bind
31716	2	7767	5	13	NULL	NULL	NULL	IgG autoantibodies	GP		bind					MDA-LDL	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_108_9_1059_s_63	12912807	30 Plasma titers of IgM and IgG autoantibodies binding to MDA-LDL and Cu-OxLDL were determined by chemiluminescence ELISA as previously described.	bind
31717	3	7767	5	13	NULL	NULL	NULL	IgM autoantibodies	GP		bind					Cu-OxLDL	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_108_9_1059_s_63	12912807	30 Plasma titers of IgM and IgG autoantibodies binding to MDA-LDL and Cu-OxLDL were determined by chemiluminescence ELISA as previously described.	bind
31718	4	7767	5	13	NULL	NULL	NULL	IgG autoantibodies	GP		bind					Cu-OxLDL	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_108_9_1059_s_63	12912807	30 Plasma titers of IgM and IgG autoantibodies binding to MDA-LDL and Cu-OxLDL were determined by chemiluminescence ELISA as previously described.	bind
24428	1	7767	6	NULL	NULL	0	NULL	IgM autoantibody	NULL		bind	NULL				MDA-LDL	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_108_9_1059_s_63	12912807	30 Plasma titers of IgM and IgG autoantibodies binding to MDA-LDL and Cu-OxLDL were determined by chemiluminescence ELISA as previously described.	bind
24429	2	7767	6	NULL	NULL	0	NULL	IgG autoantibody	NULL		bind	NULL				Cu-OxLDL	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_108_9_1059_s_63	12912807	30 Plasma titers of IgM and IgG autoantibodies binding to MDA-LDL and Cu-OxLDL were determined by chemiluminescence ELISA as previously described.	bind
31755	1	7768	5	13	NULL	NULL	NULL	TnI	GP		bind		cooperatively			actin-tropomyosin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_89_12_1184_s_159	11739284	30 This conformational change weakens the cooperative binding of TnI to actin-tropomyosin 31 and reduces the affinity of TnI for TnC, especially in the presence of Ca2+.	bind
31756	2	7768	5	13	NULL	NULL	NULL	TnI	GP		has affinity for					TnC	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_89_12_1184_s_159	11739284	30 This conformational change weakens the cooperative binding of TnI to actin-tropomyosin 31 and reduces the affinity of TnI for TnC, especially in the presence of Ca2+.	bind
24430	1	7768	6	NULL	NULL	0	NULL	TnI	NULL		bind	NULL	cooperatively			actin-tropomyosin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_89_12_1184_s_159	11739284	30 This conformational change weakens the cooperative binding of TnI to actin-tropomyosin 31 and reduces the affinity of TnI for TnC, especially in the presence of Ca2+.	bind
24431	2	7768	6	NULL	NULL	0	NULL	TnI	NULL		has affinity for	NULL				TnC	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_89_12_1184_s_159	11739284	30 This conformational change weakens the cooperative binding of TnI to actin-tropomyosin 31 and reduces the affinity of TnI for TnC, especially in the presence of Ca2+.	bind
31758	1	7769	5	13	NULL	NULL	NULL	CD4 co-receptor	GP		bind					gp120	GP				NULL		NULL	NULL	NULL	NULL	gw70_jantimicrobchemoth_54_2_333_s_37	15231762	30, 31 The binding of both CD4 and chemokine co-receptor by gp120 are the first two steps of viral entry, and the prevention of co-receptor binding, like the prevention of attachment, is an important therapeutic target.	bind
31759	2	7769	5	13	NULL	NULL	NULL	chemokine co-receptor	GP		bind					gp120	GP				NULL		NULL	NULL	NULL	NULL	gw70_jantimicrobchemoth_54_2_333_s_37	15231762	30, 31 The binding of both CD4 and chemokine co-receptor by gp120 are the first two steps of viral entry, and the prevention of co-receptor binding, like the prevention of attachment, is an important therapeutic target.	bind
31760	3	7769	5	13	NULL	NULL	NULL	viral entry	Process		leads to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jantimicrobchemoth_54_2_333_s_37	15231762	30, 31 The binding of both CD4 and chemokine co-receptor by gp120 are the first two steps of viral entry, and the prevention of co-receptor binding, like the prevention of attachment, is an important therapeutic target.	bind
31761	4	7769	5	13	NULL	NULL	NULL	viral entry	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jantimicrobchemoth_54_2_333_s_37	15231762	30, 31 The binding of both CD4 and chemokine co-receptor by gp120 are the first two steps of viral entry, and the prevention of co-receptor binding, like the prevention of attachment, is an important therapeutic target.	bind
24432	1	7769	6	NULL	NULL	0	NULL	CD4	NULL		bind	NULL				gp120	NULL				NULL		0	NULL	NULL	NULL	gw70_jantimicrobchemoth_54_2_333_s_37	15231762	30, 31 The binding of both CD4 and chemokine co-receptor by gp120 are the first two steps of viral entry, and the prevention of co-receptor binding, like the prevention of attachment, is an important therapeutic target.	bind
24433	2	7769	6	NULL	NULL	0	NULL	chemokine co-receptor	NULL		bind	NULL				gp120	NULL				NULL		0	NULL	NULL	NULL	gw70_jantimicrobchemoth_54_2_333_s_37	15231762	30, 31 The binding of both CD4 and chemokine co-receptor by gp120 are the first two steps of viral entry, and the prevention of co-receptor binding, like the prevention of attachment, is an important therapeutic target.	bind
24434	3	7769	6	NULL	NULL	0	NULL	statement 1	NULL		is the first step for	NULL				viral entry	NULL				NULL		0	NULL	NULL	NULL	gw70_jantimicrobchemoth_54_2_333_s_37	15231762	30, 31 The binding of both CD4 and chemokine co-receptor by gp120 are the first two steps of viral entry, and the prevention of co-receptor binding, like the prevention of attachment, is an important therapeutic target.	bind
24435	4	7769	6	NULL	NULL	0	NULL	statement 2	NULL		is the first step for	NULL				viral entry	NULL				NULL		0	NULL	NULL	NULL	gw70_jantimicrobchemoth_54_2_333_s_37	15231762	30, 31 The binding of both CD4 and chemokine co-receptor by gp120 are the first two steps of viral entry, and the prevention of co-receptor binding, like the prevention of attachment, is an important therapeutic target.	bind
24436	5	7769	6	10	NULL	0	NULL	co-receptor	NULL	prevention of binding of	is an important	NULL				therapeutic target	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jantimicrobchemoth_54_2_333_s_37	15231762	30, 31 The binding of both CD4 and chemokine co-receptor by gp120 are the first two steps of viral entry, and the prevention of co-receptor binding, like the prevention of attachment, is an important therapeutic target.	bind
24437	6	7769	6	NULL	NULL	0	NULL	attachment	NULL	prevention of	is an important	NULL				therapeutic target	NULL				NULL		0	NULL	NULL	NULL	gw70_jantimicrobchemoth_54_2_333_s_37	15231762	30, 31 The binding of both CD4 and chemokine co-receptor by gp120 are the first two steps of viral entry, and the prevention of co-receptor binding, like the prevention of attachment, is an important therapeutic target.	bind
31762	1	7770	5	13	NULL	NULL	NULL	cytokeratin-1	GP		bind					uPAR	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_9_1227_s_169	15044324	30,31  It has been shown that cytokeratin-1 binds to both uPAR and gC1qR, but uPAR and gC1qR do not bind to each other.	bind
31763	2	7770	5	13	NULL	NULL	NULL	cytokeratin-1	GP		bind					gC1qR	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_9_1227_s_169	15044324	30,31  It has been shown that cytokeratin-1 binds to both uPAR and gC1qR, but uPAR and gC1qR do not bind to each other.	bind
31764	3	7770	5	13	NULL	NULL	NULL	uPAR	GP		does not bind					gC1qR	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_9_1227_s_169	15044324	30,31  It has been shown that cytokeratin-1 binds to both uPAR and gC1qR, but uPAR and gC1qR do not bind to each other.	bind
24438	1	7770	6	NULL	NULL	0	NULL	cytokeratin-1	NULL		bind	NULL				uPAR	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_9_1227_s_169	15044324	30,31  It has been shown that cytokeratin-1 binds to both uPAR and gC1qR, but uPAR and gC1qR do not bind to each other.	bind
24439	2	7770	6	NULL	NULL	0	NULL	cytokeratin-1	NULL		bind	NULL				gC1qR	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_9_1227_s_169	15044324	30,31  It has been shown that cytokeratin-1 binds to both uPAR and gC1qR, but uPAR and gC1qR do not bind to each other.	bind
24440	3	7770	6	NULL	NULL	0	NULL	uPAR	NULL		does not bind	NULL				gC1qR	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_9_1227_s_169	15044324	30,31  It has been shown that cytokeratin-1 binds to both uPAR and gC1qR, but uPAR and gC1qR do not bind to each other.	bind
46846	1	7773	5	13	NULL	NULL	NULL	cells	Cell		express					CCR8	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17251_s_84	9211859	300-19 cells expressing CCR8 bound radiolabeled I-309 with high affinity (Fig.  3).	bind
46847	2	7773	5	13	NULL	NULL	NULL	statement 1	GP		bind		high affinity			I-309	GP	radiolabeled			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17251_s_84	9211859	300-19 cells expressing CCR8 bound radiolabeled I-309 with high affinity (Fig.  3).	bind
24442	2	7773	6	10	NULL	0	NULL	statement 1	NULL		bind	NULL	high affinity			I-309	NULL	radiolabeled			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_28_17251_s_84	9211859	300-19 cells expressing CCR8 bound radiolabeled I-309 with high affinity (Fig.  3).	bind
46848	1	7773	6	10	NULL	0	NULL	cells	NULL		express	NULL				CCR8	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_28_17251_s_84	9211859	300-19 cells expressing CCR8 bound radiolabeled I-309 with high affinity (Fig.  3).	bind
31768	1	7774	5	13	NULL	NULL	NULL	CAND1	GP		bind					CUL1	GP	unneddylated			NULL		NULL	NULL	NULL	NULL	gw70_nature_435_7046_1257_s_232	15988528	301, 392 398 (2003) |  Article |  PubMed |  ISI |  ChemPort |                        Zheng, J.  et al. CAND1 binds to unneddylated CUL1 and regulates the formation of SCF ubiquitin E3  ligase complex.	bind
31769	2	7774	5	13	NULL	NULL	NULL	statement 1	Process		regulates					SCF ubiquitin E3 ligase complex	GP	formation of			NULL		NULL	NULL	NULL	NULL	gw70_nature_435_7046_1257_s_232	15988528	301, 392 398 (2003) |  Article |  PubMed |  ISI |  ChemPort |                        Zheng, J.  et al. CAND1 binds to unneddylated CUL1 and regulates the formation of SCF ubiquitin E3  ligase complex.	bind
24443	1	7774	6	NULL	NULL	0	NULL	CAND1	NULL		bind	NULL				CUL1	NULL	unneddylated			NULL		0	NULL	NULL	NULL	gw70_nature_435_7046_1257_s_232	15988528	301, 392 398 (2003) |  Article |  PubMed |  ISI |  ChemPort |                        Zheng, J.  et al. CAND1 binds to unneddylated CUL1 and regulates the formation of SCF ubiquitin E3  ligase complex.	bind
24444	2	7774	6	10	NULL	0	NULL	statement 1			regulates					SCF ubiquitin E3 ligase complex		formation of			NULL		NULL	NULL	NULL	NULL	gw70_nature_435_7046_1257_s_232	15988528	301, 392 398 (2003) |  Article |  PubMed |  ISI |  ChemPort |                        Zheng, J.  et al. CAND1 binds to unneddylated CUL1 and regulates the formation of SCF ubiquitin E3  ligase complex.	bind
31770	1	7775	5	13	NULL	NULL	NULL	125I-Lac-LDL	GP		bind					Kupffer cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_6_1847_s_110	7882496	30125I-Lac-LDL binding to Kupffer cells could be inhibited up to 78% by excess unlabeled Lac-LDL at an  Ki of 1.15 plus-or-minus 0.30 nmol/L (Fig 2B  ).	bind
31771	2	7775	5	13	NULL	NULL	NULL	Lac-LDL	GP	excess unlabeled	inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_6_1847_s_110	7882496	30125I-Lac-LDL binding to Kupffer cells could be inhibited up to 78% by excess unlabeled Lac-LDL at an  Ki of 1.15 plus-or-minus 0.30 nmol/L (Fig 2B  ).	bind
24445	1	7775	6	NULL	NULL	0	NULL	125I-Lac-LDL	NULL		bind	NULL				Kupffer cells	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_91_6_1847_s_110	7882496	30125I-Lac-LDL binding to Kupffer cells could be inhibited up to 78% by excess unlabeled Lac-LDL at an  Ki of 1.15 plus-or-minus 0.30 nmol/L (Fig 2B  ).	bind
24446	2	7775	6	NULL	NULL	0	NULL	Lac-LDL	NULL	unlabeled	inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_91_6_1847_s_110	7882496	30125I-Lac-LDL binding to Kupffer cells could be inhibited up to 78% by excess unlabeled Lac-LDL at an  Ki of 1.15 plus-or-minus 0.30 nmol/L (Fig 2B  ).	bind
55545	1	7776	5	13	NULL	NULL	NULL	30K	GP		bind					p94	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31158_s_19	8537379	30K is the  first candidate to bind to and regulate p94, since the calmodulin-like  Ca -binding domains of muCL and mCL (see  Fig. 2), which are the binding sites for 30K, are highly  homologous to p94( 5) .	bind
55546	2	7776	5	13	NULL	NULL	NULL	statement 1	Process		regulates					p94	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31158_s_19	8537379	30K is the  first candidate to bind to and regulate p94, since the calmodulin-like  Ca -binding domains of muCL and mCL (see  Fig. 2), which are the binding sites for 30K, are highly  homologous to p94( 5) .	bind
55547	3	7776	5	13	NULL	NULL	NULL	muCL	GP		is a binding site for			calmodulin-like Ca -binding domains		30K	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31158_s_19	8537379	30K is the  first candidate to bind to and regulate p94, since the calmodulin-like  Ca -binding domains of muCL and mCL (see  Fig. 2), which are the binding sites for 30K, are highly  homologous to p94( 5) .	bind
55548	4	7776	5	13	NULL	NULL	NULL	mCL	GP		is a binding site for			calmodulin-like Ca -binding domains		30K	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31158_s_19	8537379	30K is the  first candidate to bind to and regulate p94, since the calmodulin-like  Ca -binding domains of muCL and mCL (see  Fig. 2), which are the binding sites for 30K, are highly  homologous to p94( 5) .	bind
55549	5	7776	5	13	NULL	NULL	NULL	statement 3	GP		is homologous to		highly			p94	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31158_s_19	8537379	30K is the  first candidate to bind to and regulate p94, since the calmodulin-like  Ca -binding domains of muCL and mCL (see  Fig. 2), which are the binding sites for 30K, are highly  homologous to p94( 5) .	bind
55550	6	7776	5	13	NULL	NULL	NULL	statement 4	GP		is homologous to		highly			p94	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31158_s_19	8537379	30K is the  first candidate to bind to and regulate p94, since the calmodulin-like  Ca -binding domains of muCL and mCL (see  Fig. 2), which are the binding sites for 30K, are highly  homologous to p94( 5) .	bind
24447	1	7776	6	NULL	NULL	0	NULL	30K	NULL		bind	NULL				p94	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31158_s_19	8537379	30K is the  first candidate to bind to and regulate p94, since the calmodulin-like  Ca -binding domains of muCL and mCL (see  Fig. 2), which are the binding sites for 30K, are highly  homologous to p94( 5) .	bind
24448	2	7776	6	NULL	NULL	0	NULL	30K	NULL		regulate	NULL				p94	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31158_s_19	8537379	30K is the  first candidate to bind to and regulate p94, since the calmodulin-like  Ca -binding domains of muCL and mCL (see  Fig. 2), which are the binding sites for 30K, are highly  homologous to p94( 5) .	bind
24569	3	7776	6	NULL	NULL	0	NULL	muCL	NULL		are homologous to	NULL		calmodulin-like Ca -binding domains		p94	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31158_s_19	8537379	30K is the  first candidate to bind to and regulate p94, since the calmodulin-like  Ca -binding domains of muCL and mCL (see  Fig. 2), which are the binding sites for 30K, are highly  homologous to p94( 5) .	bind
24570	4	7776	6	NULL	NULL	0	NULL	mCL	NULL		are homologous to	NULL		calmodulin-like Ca -binding domains		p94	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31158_s_19	8537379	30K is the  first candidate to bind to and regulate p94, since the calmodulin-like  Ca -binding domains of muCL and mCL (see  Fig. 2), which are the binding sites for 30K, are highly  homologous to p94( 5) .	bind
24950	5	7776	6	NULL	NULL	0	NULL	statement 3	NULL		is binding site for	NULL				30K	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31158_s_19	8537379	30K is the  first candidate to bind to and regulate p94, since the calmodulin-like  Ca -binding domains of muCL and mCL (see  Fig. 2), which are the binding sites for 30K, are highly  homologous to p94( 5) .	bind
24951	6	7776	6	NULL	NULL	0	NULL	statement 4	NULL		is binding site for	NULL				30K	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31158_s_19	8537379	30K is the  first candidate to bind to and regulate p94, since the calmodulin-like  Ca -binding domains of muCL and mCL (see  Fig. 2), which are the binding sites for 30K, are highly  homologous to p94( 5) .	bind
31772	1	7777	5	13	NULL	NULL	NULL	Gar1p	GP		bind			RNA binding element		snR10	NucleicAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2733_s_514	11433018	31       Bagni,C. and Lapeyre,B. (1998) Gar1p binds to the small nucleolar RNAs snR10 and snR30  in vitro through a nontypical RNA binding element.	bind
31773	2	7777	5	13	NULL	NULL	NULL	Gar1p	GP		bind			RNA binding element		snR30	NucleicAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2733_s_514	11433018	31       Bagni,C. and Lapeyre,B. (1998) Gar1p binds to the small nucleolar RNAs snR10 and snR30  in vitro through a nontypical RNA binding element.	bind
31774	3	7777	5	13	NULL	NULL	NULL	snR10	NucleicAcid		is a type of					small nucleolar RNAs	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2733_s_514	11433018	31       Bagni,C. and Lapeyre,B. (1998) Gar1p binds to the small nucleolar RNAs snR10 and snR30  in vitro through a nontypical RNA binding element.	bind
31775	4	7777	5	13	NULL	NULL	NULL	snR30	NucleicAcid		is a type of					small nucleolar RNAs	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2733_s_514	11433018	31       Bagni,C. and Lapeyre,B. (1998) Gar1p binds to the small nucleolar RNAs snR10 and snR30  in vitro through a nontypical RNA binding element.	bind
24449	1	7777	6	10	NULL	0	NULL	Gar1p	NULL		bind	NULL		nontypical RNA binding element		 snR10	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2733_s_514	11433018	31       Bagni,C. and Lapeyre,B. (1998) Gar1p binds to the small nucleolar RNAs snR10 and snR30  in vitro through a nontypical RNA binding element.	bind
24450	2	7777	6	10	NULL	0	NULL	Gar1p	NULL		bind	NULL		nontypical RNA binding element		 snR30	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2733_s_514	11433018	31       Bagni,C. and Lapeyre,B. (1998) Gar1p binds to the small nucleolar RNAs snR10 and snR30  in vitro through a nontypical RNA binding element.	bind
46849	3	7777	6	10	NULL	0	NULL	snR10	NULL		is a type of	NULL				 small nucleolar RNA	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2733_s_514	11433018	31       Bagni,C. and Lapeyre,B. (1998) Gar1p binds to the small nucleolar RNAs snR10 and snR30  in vitro through a nontypical RNA binding element.	bind
46850	4	7777	6	10	NULL	0	NULL	snR30	NULL		is a type of	NULL				small nucleolar RNA	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2733_s_514	11433018	31       Bagni,C. and Lapeyre,B. (1998) Gar1p binds to the small nucleolar RNAs snR10 and snR30  in vitro through a nontypical RNA binding element.	bind
31776	1	7778	5	13	NULL	NULL	NULL	Ets1	GP		bind		specifically			DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_20_4154_s_455	11600704	31       Bosselut,R., Levin,J., Adjadj,E. and Ghysdael,J. (1993) A single amino-acid substitution in the Ets domain alters core DNA binding specificity of Ets1 to that of the related transcription factors Elf1 and E74.	bind
31777	2	7778	5	13	NULL	NULL	NULL	Ets1	GP	single amino-acid substitution in	alters			Ets domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_20_4154_s_455	11600704	31       Bosselut,R., Levin,J., Adjadj,E. and Ghysdael,J. (1993) A single amino-acid substitution in the Ets domain alters core DNA binding specificity of Ets1 to that of the related transcription factors Elf1 and E74.	bind
31778	3	7778	5	13	NULL	NULL	NULL	Elf1	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_20_4154_s_455	11600704	31       Bosselut,R., Levin,J., Adjadj,E. and Ghysdael,J. (1993) A single amino-acid substitution in the Ets domain alters core DNA binding specificity of Ets1 to that of the related transcription factors Elf1 and E74.	bind
31779	4	7778	5	13	NULL	NULL	NULL	E74	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_20_4154_s_455	11600704	31       Bosselut,R., Levin,J., Adjadj,E. and Ghysdael,J. (1993) A single amino-acid substitution in the Ets domain alters core DNA binding specificity of Ets1 to that of the related transcription factors Elf1 and E74.	bind
24451	1	7778	6	10	NULL	0	NULL	Ets1	NULL		bind	NULL	specifically			DNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_20_4154_s_455	11600704	31       Bosselut,R., Levin,J., Adjadj,E. and Ghysdael,J. (1993) A single amino-acid substitution in the Ets domain alters core DNA binding specificity of Ets1 to that of the related transcription factors Elf1 and E74.	bind
24452	2	7778	6	10	NULL	0	NULL	Ets1	NULL	single amino-acid substitution	alters	NULL		ETS domain		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_20_4154_s_455	11600704	31       Bosselut,R., Levin,J., Adjadj,E. and Ghysdael,J. (1993) A single amino-acid substitution in the Ets domain alters core DNA binding specificity of Ets1 to that of the related transcription factors Elf1 and E74.	bind
47498	3	7778	6	10	NULL	0	NULL	Elf1	NULL		is a type of	NULL				transcription factor	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_20_4154_s_455	11600704	31       Bosselut,R., Levin,J., Adjadj,E. and Ghysdael,J. (1993) A single amino-acid substitution in the Ets domain alters core DNA binding specificity of Ets1 to that of the related transcription factors Elf1 and E74.	bind
47500	4	7778	6	10	NULL	0	NULL	E74	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_20_4154_s_455	11600704	31       Bosselut,R., Levin,J., Adjadj,E. and Ghysdael,J. (1993) A single amino-acid substitution in the Ets domain alters core DNA binding specificity of Ets1 to that of the related transcription factors Elf1 and E74.	bind
31780	1	7779	5	13	NULL	NULL	NULL	ogg1 protein	GP	Saccharomyces cerevisiae	bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_23_4583_s_400	11095666	31       Guibourt,N., Castaing,B., Van Der Kemp,P.A. and Boiteux,S. (2000) Catalytic and DNA binding properties of the ogg1 protein of Saccharomyces cerevisiae: comparison between the wild type and the K241R and K241Q active-site mutant proteins.	bind
24455	1	7779	6	13	NULL	NULL	NULL	ogg1 protein	GP	Saccharomyces cerevisiae	exhibits					catalytic activity	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_23_4583_s_400	11095666	31       Guibourt,N., Castaing,B., Van Der Kemp,P.A. and Boiteux,S. (2000) Catalytic and DNA binding properties of the ogg1 protein of Saccharomyces cerevisiae: comparison between the wild type and the K241R and K241Q active-site mutant proteins.	bind
24456	2	7779	6	NULL	NULL	0	NULL	ogg1 protein	NULL	Saccharomyces cerevisiae	bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_23_4583_s_400	11095666	31       Guibourt,N., Castaing,B., Van Der Kemp,P.A. and Boiteux,S. (2000) Catalytic and DNA binding properties of the ogg1 protein of Saccharomyces cerevisiae: comparison between the wild type and the K241R and K241Q active-site mutant proteins.	bind
31781	1	7780	5	13	NULL	NULL	NULL	C/EBP	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3311_s_337	11504868	31       Koldin,B., Suckow,M., Seydel,A., von Wilcken-Bergmann,B. and Muller-Hill,B. (1995) A comparison of the different DNA-binding specificities of the bZIP proteins C/EBP and GCN4.	bind
31782	2	7780	5	13	NULL	NULL	NULL	GCN4	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3311_s_337	11504868	31       Koldin,B., Suckow,M., Seydel,A., von Wilcken-Bergmann,B. and Muller-Hill,B. (1995) A comparison of the different DNA-binding specificities of the bZIP proteins C/EBP and GCN4.	bind
31783	3	7780	5	13	NULL	NULL	NULL	C/EBP	GP		is a type of					bZIP proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3311_s_337	11504868	31       Koldin,B., Suckow,M., Seydel,A., von Wilcken-Bergmann,B. and Muller-Hill,B. (1995) A comparison of the different DNA-binding specificities of the bZIP proteins C/EBP and GCN4.	bind
31784	4	7780	5	13	NULL	NULL	NULL	GCN4	GP		is a type of					bZIP proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3311_s_337	11504868	31       Koldin,B., Suckow,M., Seydel,A., von Wilcken-Bergmann,B. and Muller-Hill,B. (1995) A comparison of the different DNA-binding specificities of the bZIP proteins C/EBP and GCN4.	bind
24457	1	7780	6	NULL	NULL	0	NULL	C/EBP protein	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3311_s_337	11504868	31       Koldin,B., Suckow,M., Seydel,A., von Wilcken-Bergmann,B. and Muller-Hill,B. (1995) A comparison of the different DNA-binding specificities of the bZIP proteins C/EBP and GCN4.	bind
24458	2	7780	6	NULL	NULL	0	NULL	GCN4 protein	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3311_s_337	11504868	31       Koldin,B., Suckow,M., Seydel,A., von Wilcken-Bergmann,B. and Muller-Hill,B. (1995) A comparison of the different DNA-binding specificities of the bZIP proteins C/EBP and GCN4.	bind
46851	3	7780	6	10	NULL	0	NULL	C/EBP	NULL		is a type of	NULL				bZIP proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3311_s_337	11504868	31       Koldin,B., Suckow,M., Seydel,A., von Wilcken-Bergmann,B. and Muller-Hill,B. (1995) A comparison of the different DNA-binding specificities of the bZIP proteins C/EBP and GCN4.	bind
46852	4	7780	6	10	NULL	0	NULL	GCN4	NULL		is a type of	NULL				bZIP proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3311_s_337	11504868	31       Koldin,B., Suckow,M., Seydel,A., von Wilcken-Bergmann,B. and Muller-Hill,B. (1995) A comparison of the different DNA-binding specificities of the bZIP proteins C/EBP and GCN4.	bind
31785	1	7781	5	13	NULL	NULL	NULL	U2 snRNA sequences	NucleicAcid		bind					U2-specific proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_18_3841_s_318	11557816	31       Pan,Z.-Q. and Prives,C. (1989) U2 snRNA sequences that bind U2-specific proteins are dispensable for the function of U2 snRNP in splicing.	bind
31786	2	7781	5	13	NULL	NULL	NULL	U2 snRNP	NucleicAcid		function in					splicing	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_18_3841_s_318	11557816	31       Pan,Z.-Q. and Prives,C. (1989) U2 snRNA sequences that bind U2-specific proteins are dispensable for the function of U2 snRNP in splicing.	bind
31787	3	7781	5	13	NULL	NULL	NULL	statement 1	Process		dispensable for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_18_3841_s_318	11557816	31       Pan,Z.-Q. and Prives,C. (1989) U2 snRNA sequences that bind U2-specific proteins are dispensable for the function of U2 snRNP in splicing.	bind
24459	1	7781	6	NULL	NULL	0	NULL	U2 snRNA sequences	NULL		bind	NULL				U2-specific protein	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_18_3841_s_318	11557816	31       Pan,Z.-Q. and Prives,C. (1989) U2 snRNA sequences that bind U2-specific proteins are dispensable for the function of U2 snRNP in splicing.	bind
24460	2	7781	6	NULL	NULL	0	NULL	U2 snRNP	NULL		plays a role in	NULL				splicing	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_18_3841_s_318	11557816	31       Pan,Z.-Q. and Prives,C. (1989) U2 snRNA sequences that bind U2-specific proteins are dispensable for the function of U2 snRNP in splicing.	bind
24461	3	7781	6	NULL	NULL	0	NULL	statement 1	NULL		is dispensable for	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_18_3841_s_318	11557816	31       Pan,Z.-Q. and Prives,C. (1989) U2 snRNA sequences that bind U2-specific proteins are dispensable for the function of U2 snRNP in splicing.	bind
31788	1	7782	5	13	NULL	NULL	NULL	PG	GP		bind					C9 monomer	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_164_s_123	9012652	31  Because C9 has a carboxyl-terminal lysine and has lysines at amino acid positions 15 and 17 from the carboxyl terminus and since the greatest increase in PG binding occurred after the incorporation of C9 into the terminal attack complex, we hypothesized that PG bound to C9 monomer or polymer.	bind
31789	2	7782	5	13	NULL	NULL	NULL	PG	GP		bind					C9 polymer	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_164_s_123	9012652	31  Because C9 has a carboxyl-terminal lysine and has lysines at amino acid positions 15 and 17 from the carboxyl terminus and since the greatest increase in PG binding occurred after the incorporation of C9 into the terminal attack complex, we hypothesized that PG bound to C9 monomer or polymer.	bind
31790	3	7782	5	13	NULL	NULL	NULL	statement 1	Process		is alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_164_s_123	9012652	31  Because C9 has a carboxyl-terminal lysine and has lysines at amino acid positions 15 and 17 from the carboxyl terminus and since the greatest increase in PG binding occurred after the incorporation of C9 into the terminal attack complex, we hypothesized that PG bound to C9 monomer or polymer.	bind
31791	4	7782	5	13	NULL	NULL	NULL	C9	GP		contains					lysine	AminoAcid		carboxyl-terminus		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_164_s_123	9012652	31  Because C9 has a carboxyl-terminal lysine and has lysines at amino acid positions 15 and 17 from the carboxyl terminus and since the greatest increase in PG binding occurred after the incorporation of C9 into the terminal attack complex, we hypothesized that PG bound to C9 monomer or polymer.	bind
31792	5	7782	5	13	NULL	NULL	NULL	C9	GP		contains					lysine	AminoAcid		aa 15		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_164_s_123	9012652	31  Because C9 has a carboxyl-terminal lysine and has lysines at amino acid positions 15 and 17 from the carboxyl terminus and since the greatest increase in PG binding occurred after the incorporation of C9 into the terminal attack complex, we hypothesized that PG bound to C9 monomer or polymer.	bind
31793	6	7782	5	13	NULL	NULL	NULL	C9	GP		contains					lysine	AminoAcid		aa 17		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_164_s_123	9012652	31  Because C9 has a carboxyl-terminal lysine and has lysines at amino acid positions 15 and 17 from the carboxyl terminus and since the greatest increase in PG binding occurred after the incorporation of C9 into the terminal attack complex, we hypothesized that PG bound to C9 monomer or polymer.	bind
31794	7	7782	5	13	NULL	NULL	NULL	C9	GP		incorporated into					terminal attack complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_164_s_123	9012652	31  Because C9 has a carboxyl-terminal lysine and has lysines at amino acid positions 15 and 17 from the carboxyl terminus and since the greatest increase in PG binding occurred after the incorporation of C9 into the terminal attack complex, we hypothesized that PG bound to C9 monomer or polymer.	bind
31795	8	7782	5	13	NULL	NULL	NULL	statement 7	Process		increases					PG	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_164_s_123	9012652	31  Because C9 has a carboxyl-terminal lysine and has lysines at amino acid positions 15 and 17 from the carboxyl terminus and since the greatest increase in PG binding occurred after the incorporation of C9 into the terminal attack complex, we hypothesized that PG bound to C9 monomer or polymer.	bind
24462	1	7782	6	NULL	NULL	0	NULL	PG	NULL		bind	NULL				C9 monomer	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_164_s_123	9012652	31  Because C9 has a carboxyl-terminal lysine and has lysines at amino acid positions 15 and 17 from the carboxyl terminus and since the greatest increase in PG binding occurred after the incorporation of C9 into the terminal attack complex, we hypothesized that PG bound to C9 monomer or polymer.	bind
24463	2	7782	6	NULL	NULL	0	NULL	PG	NULL		bind	NULL				C9 polymer	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_164_s_123	9012652	31  Because C9 has a carboxyl-terminal lysine and has lysines at amino acid positions 15 and 17 from the carboxyl terminus and since the greatest increase in PG binding occurred after the incorporation of C9 into the terminal attack complex, we hypothesized that PG bound to C9 monomer or polymer.	bind
24464	3	7782	6	10	NULL	0	NULL	C9	NULL		contains	NULL					NULL		carboxyl-terminal lysine		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_164_s_123	9012652	31  Because C9 has a carboxyl-terminal lysine and has lysines at amino acid positions 15 and 17 from the carboxyl terminus and since the greatest increase in PG binding occurred after the incorporation of C9 into the terminal attack complex, we hypothesized that PG bound to C9 monomer or polymer.	bind
24571	4	7782	6	10	NULL	0	NULL	C9	NULL		contains	NULL					NULL		lysine at amino acid position 15 from the carboxyl terminus		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_164_s_123	9012652	31  Because C9 has a carboxyl-terminal lysine and has lysines at amino acid positions 15 and 17 from the carboxyl terminus and since the greatest increase in PG binding occurred after the incorporation of C9 into the terminal attack complex, we hypothesized that PG bound to C9 monomer or polymer.	bind
24572	5	7782	6	10	NULL	0	NULL	C9	NULL		contains	NULL					NULL		lysine at amino acid position 17 from the carboxyl terminus		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_164_s_123	9012652	31  Because C9 has a carboxyl-terminal lysine and has lysines at amino acid positions 15 and 17 from the carboxyl terminus and since the greatest increase in PG binding occurred after the incorporation of C9 into the terminal attack complex, we hypothesized that PG bound to C9 monomer or polymer.	bind
46853	6	7782	6	10	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_164_s_123	9012652	31  Because C9 has a carboxyl-terminal lysine and has lysines at amino acid positions 15 and 17 from the carboxyl terminus and since the greatest increase in PG binding occurred after the incorporation of C9 into the terminal attack complex, we hypothesized that PG bound to C9 monomer or polymer.	bind
46854	7	7782	6	10	NULL	0	NULL	C9	NULL		incorporated into	NULL				terminal attack complex	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_164_s_123	9012652	31  Because C9 has a carboxyl-terminal lysine and has lysines at amino acid positions 15 and 17 from the carboxyl terminus and since the greatest increase in PG binding occurred after the incorporation of C9 into the terminal attack complex, we hypothesized that PG bound to C9 monomer or polymer.	bind
46855	8	7782	6	10	NULL	0	NULL	statement 7	NULL		increase	NULL				PG	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_164_s_123	9012652	31  Because C9 has a carboxyl-terminal lysine and has lysines at amino acid positions 15 and 17 from the carboxyl terminus and since the greatest increase in PG binding occurred after the incorporation of C9 into the terminal attack complex, we hypothesized that PG bound to C9 monomer or polymer.	bind
31796	1	7783	5	13	NULL	NULL	NULL	HMG-1 protein	GP	recombinant	bind									KRE	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_8_937_s_201	10222341	31  Moreover, recombinant HMG-1 protein binds to KRE in the absence of poly(dI-dC).	bind
31797	2	7783	5	13	NULL	NULL	NULL	statement 1	Process		absence of					poly(dI-dC)	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_8_937_s_201	10222341	31  Moreover, recombinant HMG-1 protein binds to KRE in the absence of poly(dI-dC).	bind
24465	1	7783	6	NULL	NULL	0	NULL	HMG-1 protein	NULL	recombinant	bind	NULL					NULL			KRE	NULL		0	NULL	NULL	NULL	gw60_circulationres_84_8_937_s_201	10222341	31  Moreover, recombinant HMG-1 protein binds to KRE in the absence of poly(dI-dC).	bind
24466	2	7783	6	NULL	NULL	0	NULL	statement 1	NULL		occurs in absence of	NULL				poly(dI-dC)	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_8_937_s_201	10222341	31  Moreover, recombinant HMG-1 protein binds to KRE in the absence of poly(dI-dC).	bind
31798	1	7784	5	13	NULL	NULL	NULL	PGE1 receptor subtype	GP		bind					PGI2	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2066_s_156	9351373	31  One subtype of the PGE1 receptor binds PGI2, the other one binds PGE2.	bind
31799	2	7784	5	13	NULL	NULL	NULL	PGE1 receptor subtype	GP		bind					PGE2	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2066_s_156	9351373	31  One subtype of the PGE1 receptor binds PGI2, the other one binds PGE2.	bind
24467	1	7784	6	10	NULL	0	NULL	PGE1 receptor subtype \t			bind					PGI2					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2066_s_156	9351373	31  One subtype of the PGE1 receptor binds PGI2, the other one binds PGE2.	bind
24468	2	7784	6	10	NULL	0	NULL	PGE1 receptor subtype			bind					PGE2					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2066_s_156	9351373	31  One subtype of the PGE1 receptor binds PGI2, the other one binds PGE2.	bind
31800	1	7785	5	13	NULL	NULL	NULL	fibroblast	Cell	human;;cardiac	bind					collagen	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_10_1130_s_175	10715259	31  Our data further suggest beta1 integrin is the major receptor involved in human cardiac fibroblast binding to collagen.	bind
31801	2	7785	5	13	NULL	NULL	NULL	beta1 integrin	GP		is a type of					receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_10_1130_s_175	10715259	31  Our data further suggest beta1 integrin is the major receptor involved in human cardiac fibroblast binding to collagen.	bind
31802	3	7785	5	13	NULL	NULL	NULL	beta1 integrin	GP		is involved in					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_10_1130_s_175	10715259	31  Our data further suggest beta1 integrin is the major receptor involved in human cardiac fibroblast binding to collagen.	bind
24469	1	7785	6	10	NULL	0	NULL	fibroblast		human;;cardiac	bind					collagen					NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_10_1130_s_175	10715259	31  Our data further suggest beta1 integrin is the major receptor involved in human cardiac fibroblast binding to collagen.	bind
24470	2	7785	6	NULL	NULL	0	NULL	beta1 integrin receptor	NULL		is involved in	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_101_10_1130_s_175	10715259	31  Our data further suggest beta1 integrin is the major receptor involved in human cardiac fibroblast binding to collagen.	bind
31848	1	7786	5	13	NULL	NULL	NULL	platelets	Cell	resting	adhere to					fibrinogen	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_8_1248_s_69	9714131	31  The adhesion of resting platelets to fibrinogen was reduced by 29.4 plus-or-minus 4.1% (n=5,  P<0.001) when the binding of fibrinogen to its platelet receptor was prevented by using the specific antibody PAC1.	bind
31849	2	7786	5	13	NULL	NULL	NULL	fibrinogen	GP		bind					platelet receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_8_1248_s_69	9714131	31  The adhesion of resting platelets to fibrinogen was reduced by 29.4 plus-or-minus 4.1% (n=5,  P<0.001) when the binding of fibrinogen to its platelet receptor was prevented by using the specific antibody PAC1.	bind
31850	3	7786	5	13	NULL	NULL	NULL	PAC1 antibody	GP		prevents					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_8_1248_s_69	9714131	31  The adhesion of resting platelets to fibrinogen was reduced by 29.4 plus-or-minus 4.1% (n=5,  P<0.001) when the binding of fibrinogen to its platelet receptor was prevented by using the specific antibody PAC1.	bind
46857	4	7786	5	13	NULL	NULL	NULL	statement 3	Process		reduces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_8_1248_s_69	9714131	31  The adhesion of resting platelets to fibrinogen was reduced by 29.4 plus-or-minus 4.1% (n=5,  P<0.001) when the binding of fibrinogen to its platelet receptor was prevented by using the specific antibody PAC1.	bind
24471	1	7786	6	NULL	NULL	0	NULL	platelets 	NULL	resting	adhere to	NULL				fibrinogen	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_8_1248_s_69	9714131	31  The adhesion of resting platelets to fibrinogen was reduced by 29.4 plus-or-minus 4.1% (n=5,  P<0.001) when the binding of fibrinogen to its platelet receptor was prevented by using the specific antibody PAC1.	bind
24472	3	7786	6	10	NULL	0	NULL	antibody PAC1	NULL	specific	prevents	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_8_1248_s_69	9714131	31  The adhesion of resting platelets to fibrinogen was reduced by 29.4 plus-or-minus 4.1% (n=5,  P<0.001) when the binding of fibrinogen to its platelet receptor was prevented by using the specific antibody PAC1.	bind
46856	2	7786	6	10	NULL	0	NULL	fibrinogen	NULL		bind	NULL				platelet receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_8_1248_s_69	9714131	31  The adhesion of resting platelets to fibrinogen was reduced by 29.4 plus-or-minus 4.1% (n=5,  P<0.001) when the binding of fibrinogen to its platelet receptor was prevented by using the specific antibody PAC1.	bind
46858	4	7786	6	10	NULL	0	NULL	statement 3	NULL		reduces	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_8_1248_s_69	9714131	31  The adhesion of resting platelets to fibrinogen was reduced by 29.4 plus-or-minus 4.1% (n=5,  P<0.001) when the binding of fibrinogen to its platelet receptor was prevented by using the specific antibody PAC1.	bind
31852	1	7787	5	13	NULL	NULL	NULL	anti-LIBS1	GP	binding of	indicates					fibrinogen	GP	receptor activity of			NULL	platelet surface	NULL	NULL	NULL	NULL	gw60_circulation_93_2_229_s_63	8548893	31  Thus, anti-LIBS1 binding indicates fibrinogen receptor activity on the platelet surface.	bind
24627	1	7787	6	10	NULL	0	NULL	anti-LIBS1	NULL	binding of	indicates	NULL				fibrinogen	NULL	receptor activity of			NULL	platelet surface	NULL	NULL	NULL	NULL	gw60_circulation_93_2_229_s_63	8548893	31  Thus, anti-LIBS1 binding indicates fibrinogen receptor activity on the platelet surface.	bind
31853	1	7789	5	13	NULL	NULL	NULL	Vitronectin	GP		bind					type 1 plasminogen activator inhibitor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_3_270_s_219	9710119	31  Vitronectin binds another proteinase inhibitor, type 1 plasminogen activator inhibitor.	bind
31854	2	7789	5	13	NULL	NULL	NULL	type 1 plasminogen activator inhibitor	GP		is a type of					proteinase inhibitor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_3_270_s_219	9710119	31  Vitronectin binds another proteinase inhibitor, type 1 plasminogen activator inhibitor.	bind
24631	1	7789	6	NULL	NULL	0	NULL	vitronectin	NULL		bind	NULL				type 1 plasminogen activator inhibitor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_3_270_s_219	9710119	31  Vitronectin binds another proteinase inhibitor, type 1 plasminogen activator inhibitor.	bind
38662	2	7789	6	NULL	NULL	0	NULL	type 1 plasminogen activator inhibitor	NULL		is a type of	NULL				proteinase inhibitor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_3_270_s_219	9710119	31  Vitronectin binds another proteinase inhibitor, type 1 plasminogen activator inhibitor.	bind
31855	1	7790	5	13	NULL	NULL	NULL	BiP	GP		bind					ER stress sensors	GP		ER luminal domain		NULL	in unstressed condition	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1439_s_78	16645155	31 - 33   In unstressed condition, ER chaperone BiP binds to the ER luminal domain of 3 ER stress sensors.	bind
31856	2	7790	5	13	NULL	NULL	NULL	BiP	GP		is a type of					ER chaperone	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1439_s_78	16645155	31 - 33   In unstressed condition, ER chaperone BiP binds to the ER luminal domain of 3 ER stress sensors.	bind
24632	1	7790	6	NULL	NULL	0	NULL	BiP	NULL		bind	NULL				ER	NULL		luminal domain		NULL	unstressed condition	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1439_s_78	16645155	31 - 33   In unstressed condition, ER chaperone BiP binds to the ER luminal domain of 3 ER stress sensors.	bind
38663	2	7790	6	NULL	NULL	0	NULL	BiP	NULL		is a type of	NULL				ER chaperone	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1439_s_78	16645155	31 - 33   In unstressed condition, ER chaperone BiP binds to the ER luminal domain of 3 ER stress sensors.	bind
31857	1	7791	5	13	NULL	NULL	NULL	mAb 8A2	GP		bind					integrin receptor	GP		beta1 subunit		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_4_596_s_92	8635217	31 32 33  We have shown that mAb 8A2 binds to the beta1 subunit of the integrin receptor and enhances beta1-integrin - dependent adherence of leukocytes to cellular and matrix ligands.	bind
31858	2	7791	5	13	NULL	NULL	NULL	leukocytes	Cell		adhere to					cellular ligands	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_4_596_s_92	8635217	31 32 33  We have shown that mAb 8A2 binds to the beta1 subunit of the integrin receptor and enhances beta1-integrin - dependent adherence of leukocytes to cellular and matrix ligands.	bind
31859	3	7791	5	13	NULL	NULL	NULL	statement 2	Process		is dependent on					beta1-integrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_4_596_s_92	8635217	31 32 33  We have shown that mAb 8A2 binds to the beta1 subunit of the integrin receptor and enhances beta1-integrin - dependent adherence of leukocytes to cellular and matrix ligands.	bind
31860	4	7791	5	13	NULL	NULL	NULL	statement 1	Process		enhances					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_4_596_s_92	8635217	31 32 33  We have shown that mAb 8A2 binds to the beta1 subunit of the integrin receptor and enhances beta1-integrin - dependent adherence of leukocytes to cellular and matrix ligands.	bind
31861	5	7791	5	13	NULL	NULL	NULL	leukocytes	Cell		adhere to					matrix ligands	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_4_596_s_92	8635217	31 32 33  We have shown that mAb 8A2 binds to the beta1 subunit of the integrin receptor and enhances beta1-integrin - dependent adherence of leukocytes to cellular and matrix ligands.	bind
31862	6	7791	5	13	NULL	NULL	NULL	statement 5	Process		is dependent on					beta1-integrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_4_596_s_92	8635217	31 32 33  We have shown that mAb 8A2 binds to the beta1 subunit of the integrin receptor and enhances beta1-integrin - dependent adherence of leukocytes to cellular and matrix ligands.	bind
31863	7	7791	5	13	NULL	NULL	NULL	statement 1	Process		enhances					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_4_596_s_92	8635217	31 32 33  We have shown that mAb 8A2 binds to the beta1 subunit of the integrin receptor and enhances beta1-integrin - dependent adherence of leukocytes to cellular and matrix ligands.	bind
24633	1	7791	6	NULL	NULL	0	NULL	mAb 8A2	NULL		bind	NULL				integrin receptor	NULL		beta1 subunit		NULL		0	NULL	NULL	NULL	gw60_circulationres_78_4_596_s_92	8635217	31 32 33  We have shown that mAb 8A2 binds to the beta1 subunit of the integrin receptor and enhances beta1-integrin - dependent adherence of leukocytes to cellular and matrix ligands.	bind
24634	2	7791	6	NULL	NULL	0	NULL	leukocytes	NULL		adhers to	NULL				cellular ligands	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_78_4_596_s_92	8635217	31 32 33  We have shown that mAb 8A2 binds to the beta1 subunit of the integrin receptor and enhances beta1-integrin - dependent adherence of leukocytes to cellular and matrix ligands.	bind
24635	3	7791	6	NULL	NULL	0	NULL	leukocytes	NULL		adhere to	NULL				matrix ligands	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_78_4_596_s_92	8635217	31 32 33  We have shown that mAb 8A2 binds to the beta1 subunit of the integrin receptor and enhances beta1-integrin - dependent adherence of leukocytes to cellular and matrix ligands.	bind
24636	4	7791	6	NULL	NULL	0	NULL	statement 2	NULL		is dependent on	NULL				beta1-integrin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_78_4_596_s_92	8635217	31 32 33  We have shown that mAb 8A2 binds to the beta1 subunit of the integrin receptor and enhances beta1-integrin - dependent adherence of leukocytes to cellular and matrix ligands.	bind
24637	5	7791	6	NULL	NULL	0	NULL	statement 3	NULL		is dependent on	NULL				beta1-integrin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_78_4_596_s_92	8635217	31 32 33  We have shown that mAb 8A2 binds to the beta1 subunit of the integrin receptor and enhances beta1-integrin - dependent adherence of leukocytes to cellular and matrix ligands.	bind
46859	6	7791	6	10	NULL	0	NULL	statement 1	NULL		enhance	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_78_4_596_s_92	8635217	31 32 33  We have shown that mAb 8A2 binds to the beta1 subunit of the integrin receptor and enhances beta1-integrin - dependent adherence of leukocytes to cellular and matrix ligands.	bind
46860	7	7791	6	10	NULL	0	NULL	statement 1	NULL		enhance	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_78_4_596_s_92	8635217	31 32 33  We have shown that mAb 8A2 binds to the beta1 subunit of the integrin receptor and enhances beta1-integrin - dependent adherence of leukocytes to cellular and matrix ligands.	bind
31864	1	7792	5	13	NULL	NULL	NULL	Va receptor	GP	occupancy of	is essential for					factor Xa	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_7_2339_s_289	9337209	31 32 33 34  The occupancy of Va receptor is essential for the subsequent binding of factor Xa, whereas binding of factor VIIIa, though not essential for factor IXa binding, enhances the binding affinity of IXa by fivefold.	bind
31865	2	7792	5	13	NULL	NULL	NULL	factor VIIIa	GP	binding of	is not essential for					factor IXa	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_7_2339_s_289	9337209	31 32 33 34  The occupancy of Va receptor is essential for the subsequent binding of factor Xa, whereas binding of factor VIIIa, though not essential for factor IXa binding, enhances the binding affinity of IXa by fivefold.	bind
31866	3	7792	5	13	NULL	NULL	NULL	factor VIIIa	GP	binding of	enhances					IXa	GP	binding affinity of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_7_2339_s_289	9337209	31 32 33 34  The occupancy of Va receptor is essential for the subsequent binding of factor Xa, whereas binding of factor VIIIa, though not essential for factor IXa binding, enhances the binding affinity of IXa by fivefold.	bind
24888	1	7792	6	NULL	NULL	0	NULL	Va receptor	NULL	occupancy of	is essential for	NULL				factor Xa	NULL	binding of 			NULL		0	NULL	NULL	NULL	gw60_circulation_96_7_2339_s_289	9337209	31 32 33 34  The occupancy of Va receptor is essential for the subsequent binding of factor Xa, whereas binding of factor VIIIa, though not essential for factor IXa binding, enhances the binding affinity of IXa by fivefold.	bind
24889	2	7792	6	NULL	NULL	0	NULL	factor VIIIa	NULL	binding of	is not essential for	NULL				factor IXa	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_circulation_96_7_2339_s_289	9337209	31 32 33 34  The occupancy of Va receptor is essential for the subsequent binding of factor Xa, whereas binding of factor VIIIa, though not essential for factor IXa binding, enhances the binding affinity of IXa by fivefold.	bind
24890	3	7792	6	NULL	NULL	0	NULL	factor VIIIa	NULL	binding of	enhances	NULL				factor IXa	NULL	binding affinity of			NULL		0	NULL	NULL	NULL	gw60_circulation_96_7_2339_s_289	9337209	31 32 33 34  The occupancy of Va receptor is essential for the subsequent binding of factor Xa, whereas binding of factor VIIIa, though not essential for factor IXa binding, enhances the binding affinity of IXa by fivefold.	bind
31867	1	7793	5	13	NULL	NULL	NULL	NHE-1	GP		bind		strongly	cytoplasmic domain		calmodulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_6_962_s_223	8635246	31 50 51  Binding experiments with calmodulin-Sepharose, as well as fluorescence measurements with dansylated calmodulin, revealed that the NHE-1 cytoplasmic domain strongly binds calmodulin in a Ca2+-dependent manner.	bind
31868	2	7793	5	13	NULL	NULL	NULL	statement 1	Process		is dependent on					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_6_962_s_223	8635246	31 50 51  Binding experiments with calmodulin-Sepharose, as well as fluorescence measurements with dansylated calmodulin, revealed that the NHE-1 cytoplasmic domain strongly binds calmodulin in a Ca2+-dependent manner.	bind
24638	1	7793	6	NULL	NULL	0	NULL	NHE-1	NULL		bind	NULL	strongly	cytoplasmic domain		calmodulin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_78_6_962_s_223	8635246	31 50 51  Binding experiments with calmodulin-Sepharose, as well as fluorescence measurements with dansylated calmodulin, revealed that the NHE-1 cytoplasmic domain strongly binds calmodulin in a Ca2+-dependent manner.	bind
24639	2	7793	6	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				Ca2+	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_78_6_962_s_223	8635246	31 50 51  Binding experiments with calmodulin-Sepharose, as well as fluorescence measurements with dansylated calmodulin, revealed that the NHE-1 cytoplasmic domain strongly binds calmodulin in a Ca2+-dependent manner.	bind
31869	1	7794	5	13	NULL	NULL	NULL	fibrinogen	GP		is a type of					plasma ligand	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_8_1360_s_59	12171801	31 Abciximab was used as an anti - GP IIb/IIa agent, which blocks the binding of plasma ligands such as fibrinogen and VWF to GP IIb/IIa. 32, 33 Recent clinical investigations have revealed abciximab to be effective in preventing acute thrombotic occlusion of the coronary arteries after interventional treatment 34 and stent implantation.	bind
31870	2	7794	5	13	NULL	NULL	NULL	VWF	GP		is a type of					plasma ligand	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_8_1360_s_59	12171801	31 Abciximab was used as an anti - GP IIb/IIa agent, which blocks the binding of plasma ligands such as fibrinogen and VWF to GP IIb/IIa. 32, 33 Recent clinical investigations have revealed abciximab to be effective in preventing acute thrombotic occlusion of the coronary arteries after interventional treatment 34 and stent implantation.	bind
31871	3	7794	5	13	NULL	NULL	NULL	fibrinogen	GP		bind					GP IIb/IIa	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_8_1360_s_59	12171801	31 Abciximab was used as an anti - GP IIb/IIa agent, which blocks the binding of plasma ligands such as fibrinogen and VWF to GP IIb/IIa. 32, 33 Recent clinical investigations have revealed abciximab to be effective in preventing acute thrombotic occlusion of the coronary arteries after interventional treatment 34 and stent implantation.	bind
31872	4	7794	5	13	NULL	NULL	NULL	VWF	GP		bind					GP IIb/IIa	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_8_1360_s_59	12171801	31 Abciximab was used as an anti - GP IIb/IIa agent, which blocks the binding of plasma ligands such as fibrinogen and VWF to GP IIb/IIa. 32, 33 Recent clinical investigations have revealed abciximab to be effective in preventing acute thrombotic occlusion of the coronary arteries after interventional treatment 34 and stent implantation.	bind
31873	5	7794	5	13	NULL	NULL	NULL	Abciximab	Chemical		is a type of					anti - GP IIb/IIa agent	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_8_1360_s_59	12171801	31 Abciximab was used as an anti - GP IIb/IIa agent, which blocks the binding of plasma ligands such as fibrinogen and VWF to GP IIb/IIa. 32, 33 Recent clinical investigations have revealed abciximab to be effective in preventing acute thrombotic occlusion of the coronary arteries after interventional treatment 34 and stent implantation.	bind
31874	6	7794	5	13	NULL	NULL	NULL	Abciximab	Chemical		blocks					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_8_1360_s_59	12171801	31 Abciximab was used as an anti - GP IIb/IIa agent, which blocks the binding of plasma ligands such as fibrinogen and VWF to GP IIb/IIa. 32, 33 Recent clinical investigations have revealed abciximab to be effective in preventing acute thrombotic occlusion of the coronary arteries after interventional treatment 34 and stent implantation.	bind
31875	7	7794	5	13	NULL	NULL	NULL	Abciximab	Chemical		blocks					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_8_1360_s_59	12171801	31 Abciximab was used as an anti - GP IIb/IIa agent, which blocks the binding of plasma ligands such as fibrinogen and VWF to GP IIb/IIa. 32, 33 Recent clinical investigations have revealed abciximab to be effective in preventing acute thrombotic occlusion of the coronary arteries after interventional treatment 34 and stent implantation.	bind
31876	8	7794	5	13	NULL	NULL	NULL	Abciximab	Chemical		prevents					acute thrombotic occlusion	MedicalFinding				NULL	coronary arteries	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_8_1360_s_59	12171801	31 Abciximab was used as an anti - GP IIb/IIa agent, which blocks the binding of plasma ligands such as fibrinogen and VWF to GP IIb/IIa. 32, 33 Recent clinical investigations have revealed abciximab to be effective in preventing acute thrombotic occlusion of the coronary arteries after interventional treatment 34 and stent implantation.	bind
31877	9	7794	5	13	NULL	NULL	NULL	statement 8	Process		occurs after					interventional treatment	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_8_1360_s_59	12171801	31 Abciximab was used as an anti - GP IIb/IIa agent, which blocks the binding of plasma ligands such as fibrinogen and VWF to GP IIb/IIa. 32, 33 Recent clinical investigations have revealed abciximab to be effective in preventing acute thrombotic occlusion of the coronary arteries after interventional treatment 34 and stent implantation.	bind
31878	10	7794	5	13	NULL	NULL	NULL	statement 8	Process		occurs after					stent implantation	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_8_1360_s_59	12171801	31 Abciximab was used as an anti - GP IIb/IIa agent, which blocks the binding of plasma ligands such as fibrinogen and VWF to GP IIb/IIa. 32, 33 Recent clinical investigations have revealed abciximab to be effective in preventing acute thrombotic occlusion of the coronary arteries after interventional treatment 34 and stent implantation.	bind
24891	1	7794	6	NULL	NULL	0	NULL	fibrinogen	NULL		bind	NULL				GP IIb/IIa	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_8_1360_s_59	12171801	31 Abciximab was used as an anti - GP IIb/IIa agent, which blocks the binding of plasma ligands such as fibrinogen and VWF to GP IIb/IIa. 32, 33 Recent clinical investigations have revealed abciximab to be effective in preventing acute thrombotic occlusion of the coronary arteries after interventional treatment 34 and stent implantation.	bind
24893	2	7794	6	NULL	NULL	0	NULL	VWF	NULL		bind	NULL				GP IIb/IIa	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_8_1360_s_59	12171801	31 Abciximab was used as an anti - GP IIb/IIa agent, which blocks the binding of plasma ligands such as fibrinogen and VWF to GP IIb/IIa. 32, 33 Recent clinical investigations have revealed abciximab to be effective in preventing acute thrombotic occlusion of the coronary arteries after interventional treatment 34 and stent implantation.	bind
24894	3	7794	6	NULL	NULL	0	NULL	Abciximab	NULL		blocks	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_8_1360_s_59	12171801	31 Abciximab was used as an anti - GP IIb/IIa agent, which blocks the binding of plasma ligands such as fibrinogen and VWF to GP IIb/IIa. 32, 33 Recent clinical investigations have revealed abciximab to be effective in preventing acute thrombotic occlusion of the coronary arteries after interventional treatment 34 and stent implantation.	bind
24895	4	7794	6	NULL	NULL	0	NULL	Abciximab	NULL		blocks	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_8_1360_s_59	12171801	31 Abciximab was used as an anti - GP IIb/IIa agent, which blocks the binding of plasma ligands such as fibrinogen and VWF to GP IIb/IIa. 32, 33 Recent clinical investigations have revealed abciximab to be effective in preventing acute thrombotic occlusion of the coronary arteries after interventional treatment 34 and stent implantation.	bind
24896	5	7794	6	10	NULL	0	NULL	Abciximab	NULL		prevents	NULL				acute thrombotic occlusion	NULL				NULL	coronary arteries	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_8_1360_s_59	12171801	31 Abciximab was used as an anti - GP IIb/IIa agent, which blocks the binding of plasma ligands such as fibrinogen and VWF to GP IIb/IIa. 32, 33 Recent clinical investigations have revealed abciximab to be effective in preventing acute thrombotic occlusion of the coronary arteries after interventional treatment 34 and stent implantation.	bind
24897	6	7794	6	NULL	NULL	0	NULL	statement 5	NULL		occurs after	NULL				interventional treatment	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_8_1360_s_59	12171801	31 Abciximab was used as an anti - GP IIb/IIa agent, which blocks the binding of plasma ligands such as fibrinogen and VWF to GP IIb/IIa. 32, 33 Recent clinical investigations have revealed abciximab to be effective in preventing acute thrombotic occlusion of the coronary arteries after interventional treatment 34 and stent implantation.	bind
24898	7	7794	6	NULL	NULL	0	NULL	statement 5	NULL		occurs after	NULL				stent implantation	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_8_1360_s_59	12171801	31 Abciximab was used as an anti - GP IIb/IIa agent, which blocks the binding of plasma ligands such as fibrinogen and VWF to GP IIb/IIa. 32, 33 Recent clinical investigations have revealed abciximab to be effective in preventing acute thrombotic occlusion of the coronary arteries after interventional treatment 34 and stent implantation.	bind
38664	8	7794	6	NULL	NULL	0	NULL	fibrinogen	NULL		is a type of	NULL				plasma ligand	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_8_1360_s_59	12171801	31 Abciximab was used as an anti - GP IIb/IIa agent, which blocks the binding of plasma ligands such as fibrinogen and VWF to GP IIb/IIa. 32, 33 Recent clinical investigations have revealed abciximab to be effective in preventing acute thrombotic occlusion of the coronary arteries after interventional treatment 34 and stent implantation.	bind
38665	9	7794	6	NULL	NULL	0	NULL	vWF	NULL		is a type of	NULL				plasma ligand	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_8_1360_s_59	12171801	31 Abciximab was used as an anti - GP IIb/IIa agent, which blocks the binding of plasma ligands such as fibrinogen and VWF to GP IIb/IIa. 32, 33 Recent clinical investigations have revealed abciximab to be effective in preventing acute thrombotic occlusion of the coronary arteries after interventional treatment 34 and stent implantation.	bind
38666	10	7794	6	NULL	NULL	0	NULL	Abciximab	NULL		is a type of	NULL				anti - GP IIb/IIa agent	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_8_1360_s_59	12171801	31 Abciximab was used as an anti - GP IIb/IIa agent, which blocks the binding of plasma ligands such as fibrinogen and VWF to GP IIb/IIa. 32, 33 Recent clinical investigations have revealed abciximab to be effective in preventing acute thrombotic occlusion of the coronary arteries after interventional treatment 34 and stent implantation.	bind
31879	1	7795	5	13	NULL	NULL	NULL	CBP/p300	GP		bind					PPARalpha/RXR heterodimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_15_1861_s_39	11956132	31 Co factors that bind to the PPARalpha/RXR heterodimer include CBP/p300, PBP/TRAP220, PGC-1, and SRC-1.	bind
31880	2	7795	5	13	NULL	NULL	NULL	PBP/TRAP220	GP		bind					PPARalpha/RXR heterodimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_15_1861_s_39	11956132	31 Co factors that bind to the PPARalpha/RXR heterodimer include CBP/p300, PBP/TRAP220, PGC-1, and SRC-1.	bind
31881	3	7795	5	13	NULL	NULL	NULL	PGC-1	GP		bind					PPARalpha/RXR heterodimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_15_1861_s_39	11956132	31 Co factors that bind to the PPARalpha/RXR heterodimer include CBP/p300, PBP/TRAP220, PGC-1, and SRC-1.	bind
31882	4	7795	5	13	NULL	NULL	NULL	SRC-1	GP		bind					PPARalpha/RXR heterodimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_15_1861_s_39	11956132	31 Co factors that bind to the PPARalpha/RXR heterodimer include CBP/p300, PBP/TRAP220, PGC-1, and SRC-1.	bind
31883	5	7795	5	13	NULL	NULL	NULL	CBP/p300	GP		is a type of					co factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_15_1861_s_39	11956132	31 Co factors that bind to the PPARalpha/RXR heterodimer include CBP/p300, PBP/TRAP220, PGC-1, and SRC-1.	bind
31884	6	7795	5	13	NULL	NULL	NULL	PBP/TRAP220	GP		is a type of					co factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_15_1861_s_39	11956132	31 Co factors that bind to the PPARalpha/RXR heterodimer include CBP/p300, PBP/TRAP220, PGC-1, and SRC-1.	bind
31885	7	7795	5	13	NULL	NULL	NULL	PGC-1	GP		is a type of					co factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_15_1861_s_39	11956132	31 Co factors that bind to the PPARalpha/RXR heterodimer include CBP/p300, PBP/TRAP220, PGC-1, and SRC-1.	bind
31886	8	7795	5	13	NULL	NULL	NULL	SRC-1	GP		is a type of					co factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_15_1861_s_39	11956132	31 Co factors that bind to the PPARalpha/RXR heterodimer include CBP/p300, PBP/TRAP220, PGC-1, and SRC-1.	bind
24640	1	7795	6	NULL	NULL	0	NULL	CBP/p300	NULL		bind	NULL				PPARalpha/RXR heterodimer	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_15_1861_s_39	11956132	31 Co factors that bind to the PPARalpha/RXR heterodimer include CBP/p300, PBP/TRAP220, PGC-1, and SRC-1.	bind
24641	2	7795	6	NULL	NULL	0	NULL	PBP/TRAP220	NULL		bind	NULL				PPARalpha/RXR heterodimer	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_15_1861_s_39	11956132	31 Co factors that bind to the PPARalpha/RXR heterodimer include CBP/p300, PBP/TRAP220, PGC-1, and SRC-1.	bind
24642	3	7795	6	NULL	NULL	0	NULL	PGC-1	NULL		bind	NULL				PPARalpha/RXR heterodimer	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_15_1861_s_39	11956132	31 Co factors that bind to the PPARalpha/RXR heterodimer include CBP/p300, PBP/TRAP220, PGC-1, and SRC-1.	bind
24643	4	7795	6	NULL	NULL	0	NULL	SRC-1	NULL		bind	NULL				PPARalpha/RXR heterodimer	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_15_1861_s_39	11956132	31 Co factors that bind to the PPARalpha/RXR heterodimer include CBP/p300, PBP/TRAP220, PGC-1, and SRC-1.	bind
38667	5	7795	6	NULL	NULL	0	NULL	CBP/p300	NULL		is a type of	NULL				cofactor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_15_1861_s_39	11956132	31 Co factors that bind to the PPARalpha/RXR heterodimer include CBP/p300, PBP/TRAP220, PGC-1, and SRC-1.	bind
38668	6	7795	6	NULL	NULL	0	NULL	PBP/TRAP220	NULL		is a type of	NULL				cofactor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_15_1861_s_39	11956132	31 Co factors that bind to the PPARalpha/RXR heterodimer include CBP/p300, PBP/TRAP220, PGC-1, and SRC-1.	bind
38669	7	7795	6	NULL	NULL	0	NULL	PGC-1	NULL		is a type of	NULL				cofactor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_15_1861_s_39	11956132	31 Co factors that bind to the PPARalpha/RXR heterodimer include CBP/p300, PBP/TRAP220, PGC-1, and SRC-1.	bind
38670	8	7795	6	NULL	NULL	0	NULL	SRC-1	NULL		is a type of	NULL				cofactor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_15_1861_s_39	11956132	31 Co factors that bind to the PPARalpha/RXR heterodimer include CBP/p300, PBP/TRAP220, PGC-1, and SRC-1.	bind
31887	1	7796	5	13	NULL	NULL	NULL	estrogen	Chemical		induces					IGF-1R mRNA	NucleicAcid	downregulation of			NULL	rat aortic VSMCs	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_67	14604834	31 Estrogen-induced downregulation of IGF-1R mRNA and protein in rat aortic VSMCs was mediated by the inhibition of SP-1 binding to the IGF-1R promoter.	bind
31888	2	7796	5	13	NULL	NULL	NULL	estrogen	Chemical		induces					IGF-1R protein	GP	downregulation of			NULL	rat aortic VSMCs	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_67	14604834	31 Estrogen-induced downregulation of IGF-1R mRNA and protein in rat aortic VSMCs was mediated by the inhibition of SP-1 binding to the IGF-1R promoter.	bind
31889	3	7796	5	13	NULL	NULL	NULL	SP-1	GP		bind					IGF-1R	GP			promoter	NULL	rat aortic VSMCs	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_67	14604834	31 Estrogen-induced downregulation of IGF-1R mRNA and protein in rat aortic VSMCs was mediated by the inhibition of SP-1 binding to the IGF-1R promoter.	bind
31890	4	7796	5	13	NULL	NULL	NULL	statement 3	Process	inhibition of	mediates					statement 1	Process				NULL	rat aortic VSMCs	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_67	14604834	31 Estrogen-induced downregulation of IGF-1R mRNA and protein in rat aortic VSMCs was mediated by the inhibition of SP-1 binding to the IGF-1R promoter.	bind
31891	5	7796	5	13	NULL	NULL	NULL	statement 3	Process	inhibition of	mediates					statement 2	Process				NULL	rat aortic VSMCs	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_67	14604834	31 Estrogen-induced downregulation of IGF-1R mRNA and protein in rat aortic VSMCs was mediated by the inhibition of SP-1 binding to the IGF-1R promoter.	bind
24644	1	7796	6	10	NULL	0	NULL	SP-1			bind					IGF-1R				promoter	NULL	rat aortic VSMCs	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_67	14604834	31 Estrogen-induced downregulation of IGF-1R mRNA and protein in rat aortic VSMCs was mediated by the inhibition of SP-1 binding to the IGF-1R promoter.	bind
24645	2	7796	6	NULL	NULL	0	NULL	estrogen	NULL		induces	NULL				IGF-1R mRNA	NULL	downregulation of			NULL	rat aortic VSMCs	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_67	14604834	31 Estrogen-induced downregulation of IGF-1R mRNA and protein in rat aortic VSMCs was mediated by the inhibition of SP-1 binding to the IGF-1R promoter.	bind
24646	3	7796	6	NULL	NULL	0	NULL	estrogen	NULL		induces	NULL				IGF-1R protein	NULL	downregulation of			NULL	rat aortic VSMCs	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_67	14604834	31 Estrogen-induced downregulation of IGF-1R mRNA and protein in rat aortic VSMCs was mediated by the inhibition of SP-1 binding to the IGF-1R promoter.	bind
24647	4	7796	6	10	NULL	0	NULL	statement 2			is mediated by					statement 1		inhibiton of			NULL	rat aortic VSMCs	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_67	14604834	31 Estrogen-induced downregulation of IGF-1R mRNA and protein in rat aortic VSMCs was mediated by the inhibition of SP-1 binding to the IGF-1R promoter.	bind
24648	5	7796	6	10	NULL	0	NULL	statement 3			is mediated by					statement 1		inhibiton of			NULL	rat aortic VSMCs	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_67	14604834	31 Estrogen-induced downregulation of IGF-1R mRNA and protein in rat aortic VSMCs was mediated by the inhibition of SP-1 binding to the IGF-1R promoter.	bind
31892	1	7797	5	13	NULL	NULL	NULL	TNF-alpha	GP		stimulates					endothelial proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_9_880_s_256	16166554	31 Our EMSA indicated that LA suppressed not only NF-kappaB binding but also SP-1 binding of TNF-alpha - or IL-1beta - stimulated endothelial proteins to the DNA.	bind
31893	2	7797	5	13	NULL	NULL	NULL	IL-1beta 	GP		stimulates					endothelial proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_9_880_s_256	16166554	31 Our EMSA indicated that LA suppressed not only NF-kappaB binding but also SP-1 binding of TNF-alpha - or IL-1beta - stimulated endothelial proteins to the DNA.	bind
31894	5	7797	5	13	NULL	NULL	NULL	SP-1	GP		bind					statement 3	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_9_880_s_256	16166554	31 Our EMSA indicated that LA suppressed not only NF-kappaB binding but also SP-1 binding of TNF-alpha - or IL-1beta - stimulated endothelial proteins to the DNA.	bind
31895	6	7797	5	13	NULL	NULL	NULL	SP-1	GP		bind					statement 4	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_9_880_s_256	16166554	31 Our EMSA indicated that LA suppressed not only NF-kappaB binding but also SP-1 binding of TNF-alpha - or IL-1beta - stimulated endothelial proteins to the DNA.	bind
31896	7	7797	5	13	NULL	NULL	NULL	NF-kappaB	GP		bind					statement 3	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_9_880_s_256	16166554	31 Our EMSA indicated that LA suppressed not only NF-kappaB binding but also SP-1 binding of TNF-alpha - or IL-1beta - stimulated endothelial proteins to the DNA.	bind
31897	8	7797	5	13	NULL	NULL	NULL	NF-kappaB	GP		bind					statement 4	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_9_880_s_256	16166554	31 Our EMSA indicated that LA suppressed not only NF-kappaB binding but also SP-1 binding of TNF-alpha - or IL-1beta - stimulated endothelial proteins to the DNA.	bind
31898	9	7797	5	13	NULL	NULL	NULL	LA	Chemical		supress					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_9_880_s_256	16166554	31 Our EMSA indicated that LA suppressed not only NF-kappaB binding but also SP-1 binding of TNF-alpha - or IL-1beta - stimulated endothelial proteins to the DNA.	bind
31899	10	7797	5	13	NULL	NULL	NULL	LA	Chemical		supress					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_9_880_s_256	16166554	31 Our EMSA indicated that LA suppressed not only NF-kappaB binding but also SP-1 binding of TNF-alpha - or IL-1beta - stimulated endothelial proteins to the DNA.	bind
31900	11	7797	5	13	NULL	NULL	NULL	LA	Chemical		supress					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_9_880_s_256	16166554	31 Our EMSA indicated that LA suppressed not only NF-kappaB binding but also SP-1 binding of TNF-alpha - or IL-1beta - stimulated endothelial proteins to the DNA.	bind
31901	12	7797	5	13	NULL	NULL	NULL	LA	Chemical		supress					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_9_880_s_256	16166554	31 Our EMSA indicated that LA suppressed not only NF-kappaB binding but also SP-1 binding of TNF-alpha - or IL-1beta - stimulated endothelial proteins to the DNA.	bind
46861	3	7797	5	13	NULL	NULL	NULL	statement 1	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_9_880_s_256	16166554	31 Our EMSA indicated that LA suppressed not only NF-kappaB binding but also SP-1 binding of TNF-alpha - or IL-1beta - stimulated endothelial proteins to the DNA.	bind
46862	4	7797	5	13	NULL	NULL	NULL	statement 2	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_9_880_s_256	16166554	31 Our EMSA indicated that LA suppressed not only NF-kappaB binding but also SP-1 binding of TNF-alpha - or IL-1beta - stimulated endothelial proteins to the DNA.	bind
24649	1	7797	6	10	NULL	0	NULL	TNF-alpha	NULL		stimulate	NULL				endothelial protein	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_9_880_s_256	16166554	31 Our EMSA indicated that LA suppressed not only NF-kappaB binding but also SP-1 binding of TNF-alpha - or IL-1beta - stimulated endothelial proteins to the DNA.	bind
24650	2	7797	6	10	NULL	0	NULL	IL-1beta	NULL		stimulate	NULL				endothelial protein	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_9_880_s_256	16166554	31 Our EMSA indicated that LA suppressed not only NF-kappaB binding but also SP-1 binding of TNF-alpha - or IL-1beta - stimulated endothelial proteins to the DNA.	bind
24651	5	7797	6	10	NULL	0	NULL	NF-kappaB	NULL		bind	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_9_880_s_256	16166554	31 Our EMSA indicated that LA suppressed not only NF-kappaB binding but also SP-1 binding of TNF-alpha - or IL-1beta - stimulated endothelial proteins to the DNA.	bind
24652	6	7797	6	10	NULL	0	NULL	NF-kappaB	NULL		bind	NULL				statement 4	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_9_880_s_256	16166554	31 Our EMSA indicated that LA suppressed not only NF-kappaB binding but also SP-1 binding of TNF-alpha - or IL-1beta - stimulated endothelial proteins to the DNA.	bind
24653	7	7797	6	10	NULL	0	NULL	Sp1	NULL		bind	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_9_880_s_256	16166554	31 Our EMSA indicated that LA suppressed not only NF-kappaB binding but also SP-1 binding of TNF-alpha - or IL-1beta - stimulated endothelial proteins to the DNA.	bind
24654	8	7797	6	10	NULL	0	NULL	Sp1	NULL		bind	NULL				statement 4	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_9_880_s_256	16166554	31 Our EMSA indicated that LA suppressed not only NF-kappaB binding but also SP-1 binding of TNF-alpha - or IL-1beta - stimulated endothelial proteins to the DNA.	bind
38750	9	7797	6	10	NULL	0	NULL	LA	NULL		suppresses	NULL				statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_9_880_s_256	16166554	31 Our EMSA indicated that LA suppressed not only NF-kappaB binding but also SP-1 binding of TNF-alpha - or IL-1beta - stimulated endothelial proteins to the DNA.	bind
38751	10	7797	6	10	NULL	0	NULL	LA	NULL		suppresses	NULL				statement 6	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_9_880_s_256	16166554	31 Our EMSA indicated that LA suppressed not only NF-kappaB binding but also SP-1 binding of TNF-alpha - or IL-1beta - stimulated endothelial proteins to the DNA.	bind
38752	11	7797	6	10	NULL	0	NULL	LA	NULL		suppresses	NULL				statement 7	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_9_880_s_256	16166554	31 Our EMSA indicated that LA suppressed not only NF-kappaB binding but also SP-1 binding of TNF-alpha - or IL-1beta - stimulated endothelial proteins to the DNA.	bind
38753	12	7797	6	10	NULL	0	NULL	LA	NULL		suppresses	NULL				statement 8	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_9_880_s_256	16166554	31 Our EMSA indicated that LA suppressed not only NF-kappaB binding but also SP-1 binding of TNF-alpha - or IL-1beta - stimulated endothelial proteins to the DNA.	bind
46863	3	7797	6	10	NULL	0	NULL	statement 1	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_9_880_s_256	16166554	31 Our EMSA indicated that LA suppressed not only NF-kappaB binding but also SP-1 binding of TNF-alpha - or IL-1beta - stimulated endothelial proteins to the DNA.	bind
46864	4	7797	6	10	NULL	0	NULL	statement 2	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_9_880_s_256	16166554	31 Our EMSA indicated that LA suppressed not only NF-kappaB binding but also SP-1 binding of TNF-alpha - or IL-1beta - stimulated endothelial proteins to the DNA.	bind
31902	1	7798	5	13	NULL	NULL	NULL	tetracycline repression system	Process		induces					FAK	GP	expression of			NULL	FAK-null fibroblasts	NULL	NULL	NULL	NULL	gw70_circulationres_98_3_378_s_191	16397143	31 Surprisingly, induced expression of FAK using a tetracycline repression system in FAK-null fibroblasts led to a marked expression of LPP consistent with FAK regulating the expression of LPP, as it has been reported to induce expression of the homeodomain protein Prx1, 32 and Prx1 has been shown to increase SRF binding to CArG elements before the recruitment of myocardin in SMCs. 33 The role of FAK and LPP in nonmotile cells is less clear.	bind
31903	2	7798	5	13	NULL	NULL	NULL	statement 1	Process		leads to					LPP	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_378_s_191	16397143	31 Surprisingly, induced expression of FAK using a tetracycline repression system in FAK-null fibroblasts led to a marked expression of LPP consistent with FAK regulating the expression of LPP, as it has been reported to induce expression of the homeodomain protein Prx1, 32 and Prx1 has been shown to increase SRF binding to CArG elements before the recruitment of myocardin in SMCs. 33 The role of FAK and LPP in nonmotile cells is less clear.	bind
31904	3	7798	5	13	NULL	NULL	NULL	FAK	GP		regulates					LPP	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_378_s_191	16397143	31 Surprisingly, induced expression of FAK using a tetracycline repression system in FAK-null fibroblasts led to a marked expression of LPP consistent with FAK regulating the expression of LPP, as it has been reported to induce expression of the homeodomain protein Prx1, 32 and Prx1 has been shown to increase SRF binding to CArG elements before the recruitment of myocardin in SMCs. 33 The role of FAK and LPP in nonmotile cells is less clear.	bind
31905	4	7798	5	13	NULL	NULL	NULL	statement 2	Process		consistent with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_378_s_191	16397143	31 Surprisingly, induced expression of FAK using a tetracycline repression system in FAK-null fibroblasts led to a marked expression of LPP consistent with FAK regulating the expression of LPP, as it has been reported to induce expression of the homeodomain protein Prx1, 32 and Prx1 has been shown to increase SRF binding to CArG elements before the recruitment of myocardin in SMCs. 33 The role of FAK and LPP in nonmotile cells is less clear.	bind
31906	5	7798	5	13	NULL	NULL	NULL	FAK	GP		induces					Prx1	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_378_s_191	16397143	31 Surprisingly, induced expression of FAK using a tetracycline repression system in FAK-null fibroblasts led to a marked expression of LPP consistent with FAK regulating the expression of LPP, as it has been reported to induce expression of the homeodomain protein Prx1, 32 and Prx1 has been shown to increase SRF binding to CArG elements before the recruitment of myocardin in SMCs. 33 The role of FAK and LPP in nonmotile cells is less clear.	bind
31907	6	7798	5	13	NULL	NULL	NULL	Prx1	GP		is a type of					homeodomain protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_378_s_191	16397143	31 Surprisingly, induced expression of FAK using a tetracycline repression system in FAK-null fibroblasts led to a marked expression of LPP consistent with FAK regulating the expression of LPP, as it has been reported to induce expression of the homeodomain protein Prx1, 32 and Prx1 has been shown to increase SRF binding to CArG elements before the recruitment of myocardin in SMCs. 33 The role of FAK and LPP in nonmotile cells is less clear.	bind
31908	7	7798	5	13	NULL	NULL	NULL	SRF	GP		bind									CArG elements	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_378_s_191	16397143	31 Surprisingly, induced expression of FAK using a tetracycline repression system in FAK-null fibroblasts led to a marked expression of LPP consistent with FAK regulating the expression of LPP, as it has been reported to induce expression of the homeodomain protein Prx1, 32 and Prx1 has been shown to increase SRF binding to CArG elements before the recruitment of myocardin in SMCs. 33 The role of FAK and LPP in nonmotile cells is less clear.	bind
31909	8	7798	5	13	NULL	NULL	NULL	Prx1	GP		increases					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_378_s_191	16397143	31 Surprisingly, induced expression of FAK using a tetracycline repression system in FAK-null fibroblasts led to a marked expression of LPP consistent with FAK regulating the expression of LPP, as it has been reported to induce expression of the homeodomain protein Prx1, 32 and Prx1 has been shown to increase SRF binding to CArG elements before the recruitment of myocardin in SMCs. 33 The role of FAK and LPP in nonmotile cells is less clear.	bind
31910	9	7798	5	13	NULL	NULL	NULL	myocardin	GP		is recruited to					SMCs	Cell				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_378_s_191	16397143	31 Surprisingly, induced expression of FAK using a tetracycline repression system in FAK-null fibroblasts led to a marked expression of LPP consistent with FAK regulating the expression of LPP, as it has been reported to induce expression of the homeodomain protein Prx1, 32 and Prx1 has been shown to increase SRF binding to CArG elements before the recruitment of myocardin in SMCs. 33 The role of FAK and LPP in nonmotile cells is less clear.	bind
31911	10	7798	5	13	NULL	NULL	NULL	statement 8	Process		occurs before					statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_378_s_191	16397143	31 Surprisingly, induced expression of FAK using a tetracycline repression system in FAK-null fibroblasts led to a marked expression of LPP consistent with FAK regulating the expression of LPP, as it has been reported to induce expression of the homeodomain protein Prx1, 32 and Prx1 has been shown to increase SRF binding to CArG elements before the recruitment of myocardin in SMCs. 33 The role of FAK and LPP in nonmotile cells is less clear.	bind
24899	1	7798	6	NULL	NULL	0	NULL	SRF	NULL		bind	NULL					NULL			CArG element	NULL		0	NULL	NULL	NULL	gw70_circulationres_98_3_378_s_191	16397143	31 Surprisingly, induced expression of FAK using a tetracycline repression system in FAK-null fibroblasts led to a marked expression of LPP consistent with FAK regulating the expression of LPP, as it has been reported to induce expression of the homeodomain protein Prx1, 32 and Prx1 has been shown to increase SRF binding to CArG elements before the recruitment of myocardin in SMCs. 33 The role of FAK and LPP in nonmotile cells is less clear.	bind
24900	2	7798	6	NULL	NULL	0	NULL	Prx1	NULL		increase	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_3_378_s_191	16397143	31 Surprisingly, induced expression of FAK using a tetracycline repression system in FAK-null fibroblasts led to a marked expression of LPP consistent with FAK regulating the expression of LPP, as it has been reported to induce expression of the homeodomain protein Prx1, 32 and Prx1 has been shown to increase SRF binding to CArG elements before the recruitment of myocardin in SMCs. 33 The role of FAK and LPP in nonmotile cells is less clear.	bind
24901	3	7798	6	NULL	NULL	0	NULL	myocardin	NULL		is recruited on	NULL				SMC	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_3_378_s_191	16397143	31 Surprisingly, induced expression of FAK using a tetracycline repression system in FAK-null fibroblasts led to a marked expression of LPP consistent with FAK regulating the expression of LPP, as it has been reported to induce expression of the homeodomain protein Prx1, 32 and Prx1 has been shown to increase SRF binding to CArG elements before the recruitment of myocardin in SMCs. 33 The role of FAK and LPP in nonmotile cells is less clear.	bind
24902	4	7798	6	NULL	NULL	0	NULL	statement 1	NULL		occurs before	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_3_378_s_191	16397143	31 Surprisingly, induced expression of FAK using a tetracycline repression system in FAK-null fibroblasts led to a marked expression of LPP consistent with FAK regulating the expression of LPP, as it has been reported to induce expression of the homeodomain protein Prx1, 32 and Prx1 has been shown to increase SRF binding to CArG elements before the recruitment of myocardin in SMCs. 33 The role of FAK and LPP in nonmotile cells is less clear.	bind
24903	5	7798	6	NULL	NULL	0	NULL	statement 8	NULL		leads to	NULL				LPP	NULL	expression of			NULL	FAK-null fibroblasts	NULL	NULL	NULL	NULL	gw70_circulationres_98_3_378_s_191	16397143	31 Surprisingly, induced expression of FAK using a tetracycline repression system in FAK-null fibroblasts led to a marked expression of LPP consistent with FAK regulating the expression of LPP, as it has been reported to induce expression of the homeodomain protein Prx1, 32 and Prx1 has been shown to increase SRF binding to CArG elements before the recruitment of myocardin in SMCs. 33 The role of FAK and LPP in nonmotile cells is less clear.	bind
24904	6	7798	6	NULL	NULL	0	NULL	FAK	NULL		regulates	NULL				LPP	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_circulationres_98_3_378_s_191	16397143	31 Surprisingly, induced expression of FAK using a tetracycline repression system in FAK-null fibroblasts led to a marked expression of LPP consistent with FAK regulating the expression of LPP, as it has been reported to induce expression of the homeodomain protein Prx1, 32 and Prx1 has been shown to increase SRF binding to CArG elements before the recruitment of myocardin in SMCs. 33 The role of FAK and LPP in nonmotile cells is less clear.	bind
24905	7	7798	6	NULL	NULL	0	NULL	FAK	NULL		induce	NULL				Prx1	NULL	expression of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_378_s_191	16397143	31 Surprisingly, induced expression of FAK using a tetracycline repression system in FAK-null fibroblasts led to a marked expression of LPP consistent with FAK regulating the expression of LPP, as it has been reported to induce expression of the homeodomain protein Prx1, 32 and Prx1 has been shown to increase SRF binding to CArG elements before the recruitment of myocardin in SMCs. 33 The role of FAK and LPP in nonmotile cells is less clear.	bind
38754	8	7798	6	NULL	NULL	0	NULL	tetracycline repression system	NULL		induces	NULL				FAK	NULL	expression of			NULL	FAK-null fibroblasts	0	NULL	NULL	NULL	gw70_circulationres_98_3_378_s_191	16397143	31 Surprisingly, induced expression of FAK using a tetracycline repression system in FAK-null fibroblasts led to a marked expression of LPP consistent with FAK regulating the expression of LPP, as it has been reported to induce expression of the homeodomain protein Prx1, 32 and Prx1 has been shown to increase SRF binding to CArG elements before the recruitment of myocardin in SMCs. 33 The role of FAK and LPP in nonmotile cells is less clear.	bind
38755	9	7798	6	NULL	NULL	0	NULL	Prx1	NULL		is a type of	NULL				homeodomain protein	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_3_378_s_191	16397143	31 Surprisingly, induced expression of FAK using a tetracycline repression system in FAK-null fibroblasts led to a marked expression of LPP consistent with FAK regulating the expression of LPP, as it has been reported to induce expression of the homeodomain protein Prx1, 32 and Prx1 has been shown to increase SRF binding to CArG elements before the recruitment of myocardin in SMCs. 33 The role of FAK and LPP in nonmotile cells is less clear.	bind
31912	1	7799	5	13	NULL	NULL	NULL	decorin	GP		bind					hydroxyapatite	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2391_s_148	15472131	31 The binding of decorin to hydroxyapatite was demonstrated at concentrations >1 mg/mL.	bind
24655	1	7799	6	NULL	NULL	0	NULL	decorin	NULL		bind	NULL				hydroxyapatite	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2391_s_148	15472131	31 The binding of decorin to hydroxyapatite was demonstrated at concentrations >1 mg/mL.	bind
31913	1	7801	5	13	NULL	NULL	NULL	ATP	Chemical		bind					receptor	GP		TK domain		NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_3_423_s_198	16027270	31 TKI inhibition works via competitive inhibition of the binding of ATP to the TK domain of the receptor, which results in attenuated autophosphorylation.	bind
31914	2	7801	5	13	NULL	NULL	NULL	TKI	GP		inhibits		competitively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_3_423_s_198	16027270	31 TKI inhibition works via competitive inhibition of the binding of ATP to the TK domain of the receptor, which results in attenuated autophosphorylation.	bind
31915	3	7801	5	13	NULL	NULL	NULL	statement 2	Process		results in					autophosphorylation	Process	attenuated			NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_3_423_s_198	16027270	31 TKI inhibition works via competitive inhibition of the binding of ATP to the TK domain of the receptor, which results in attenuated autophosphorylation.	bind
24656	1	7801	6	NULL	NULL	0	NULL	ATP	NULL		bind	NULL				receptor	NULL		TK domain		NULL		0	NULL	NULL	NULL	gw70_circulation_112_3_423_s_198	16027270	31 TKI inhibition works via competitive inhibition of the binding of ATP to the TK domain of the receptor, which results in attenuated autophosphorylation.	bind
24657	2	7801	6	NULL	NULL	0	NULL	TKI	NULL		inhibits	NULL	competitively			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_112_3_423_s_198	16027270	31 TKI inhibition works via competitive inhibition of the binding of ATP to the TK domain of the receptor, which results in attenuated autophosphorylation.	bind
24658	3	7801	6	NULL	NULL	0	NULL	statement 2	NULL		results in	NULL				autophosphorylation	NULL	attenuated			NULL		0	NULL	NULL	NULL	gw70_circulation_112_3_423_s_198	16027270	31 TKI inhibition works via competitive inhibition of the binding of ATP to the TK domain of the receptor, which results in attenuated autophosphorylation.	bind
47121	1	7802	5	13	NULL	NULL	NULL	HgCl2	Chemical		bind					humic acids	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5416_939_s_148	0010320369	31, 233 (1997)  [CrossRef] [ISI];   H. Biester and H. Zimmer,       ibid. 32, 2755 (1998)] have demonstrated that Hg degrees  is the only Hg species that has significant thermal desorption below 100 degrees C, whereas HgCl2 and Hg bound to humic acids have maximum Hg releases at much higher temperatures (200 degrees  to 300 degrees C).	bind
47122	1	7802	5	13	NULL	NULL	NULL	Hg	Chemical		bind					humic acids	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5416_939_s_148	0010320369	31, 233 (1997)  [CrossRef] [ISI];   H. Biester and H. Zimmer,       ibid. 32, 2755 (1998)] have demonstrated that Hg degrees  is the only Hg species that has significant thermal desorption below 100 degrees C, whereas HgCl2 and Hg bound to humic acids have maximum Hg releases at much higher temperatures (200 degrees  to 300 degrees C).	bind
24659	1	7802	6	NULL	NULL	0	NULL	HgCl2	NULL		bind	NULL				humic acids	NULL				NULL		0	NULL	NULL	NULL	gw60_science_284_5416_939_s_148	0010320369	31, 233 (1997)  [CrossRef] [ISI];   H. Biester and H. Zimmer,       ibid. 32, 2755 (1998)] have demonstrated that Hg degrees  is the only Hg species that has significant thermal desorption below 100 degrees C, whereas HgCl2 and Hg bound to humic acids have maximum Hg releases at much higher temperatures (200 degrees  to 300 degrees C).	bind
24660	2	7802	6	NULL	NULL	0	NULL	Hg	NULL		bind	NULL				humic acids	NULL				NULL		0	NULL	NULL	NULL	gw60_science_284_5416_939_s_148	0010320369	31, 233 (1997)  [CrossRef] [ISI];   H. Biester and H. Zimmer,       ibid. 32, 2755 (1998)] have demonstrated that Hg degrees  is the only Hg species that has significant thermal desorption below 100 degrees C, whereas HgCl2 and Hg bound to humic acids have maximum Hg releases at much higher temperatures (200 degrees  to 300 degrees C).	bind
31916	1	7803	5	13	NULL	NULL	NULL	serum	OrganismPart		induces					TF	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_163	12600889	31, 32 In contrast, the SRR mediates induction of TF expression by serum, lipoproteins, or shear stress 12, 13, 32 and contains three Sp1 and one Egr-1 binding sites.	bind
31917	2	7803	5	13	NULL	NULL	NULL	lipoproteins	GP		induces					TF	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_163	12600889	31, 32 In contrast, the SRR mediates induction of TF expression by serum, lipoproteins, or shear stress 12, 13, 32 and contains three Sp1 and one Egr-1 binding sites.	bind
31918	3	7803	5	13	NULL	NULL	NULL	shear stress			induces					TF	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_163	12600889	31, 32 In contrast, the SRR mediates induction of TF expression by serum, lipoproteins, or shear stress 12, 13, 32 and contains three Sp1 and one Egr-1 binding sites.	bind
31919	4	7803	5	13	NULL	NULL	NULL				mediates				SRR	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_163	12600889	31, 32 In contrast, the SRR mediates induction of TF expression by serum, lipoproteins, or shear stress 12, 13, 32 and contains three Sp1 and one Egr-1 binding sites.	bind
31920	5	7803	5	13	NULL	NULL	NULL				mediates				SRR	statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_163	12600889	31, 32 In contrast, the SRR mediates induction of TF expression by serum, lipoproteins, or shear stress 12, 13, 32 and contains three Sp1 and one Egr-1 binding sites.	bind
31921	6	7803	5	13	NULL	NULL	NULL				mediates				SRR	statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_163	12600889	31, 32 In contrast, the SRR mediates induction of TF expression by serum, lipoproteins, or shear stress 12, 13, 32 and contains three Sp1 and one Egr-1 binding sites.	bind
31922	7	7803	5	NULL	NULL	0	NULL		NULL		contains	NULL			SRR		NULL			Egr-1 binding sites	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_163	12600889	31, 32 In contrast, the SRR mediates induction of TF expression by serum, lipoproteins, or shear stress 12, 13, 32 and contains three Sp1 and one Egr-1 binding sites.	bind
31923	8	7803	5	NULL	NULL	0	NULL		NULL		contains	NULL			SRR		NULL			Sp1 binding sites	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_163	12600889	31, 32 In contrast, the SRR mediates induction of TF expression by serum, lipoproteins, or shear stress 12, 13, 32 and contains three Sp1 and one Egr-1 binding sites.	bind
24661	1	7803	6	NULL	NULL	0	NULL	serum	NULL		induces	NULL				TF	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_163	12600889	31, 32 In contrast, the SRR mediates induction of TF expression by serum, lipoproteins, or shear stress 12, 13, 32 and contains three Sp1 and one Egr-1 binding sites.	bind
24662	2	7803	6	NULL	NULL	0	NULL		NULL		mediates	NULL			SRR	statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_163	12600889	31, 32 In contrast, the SRR mediates induction of TF expression by serum, lipoproteins, or shear stress 12, 13, 32 and contains three Sp1 and one Egr-1 binding sites.	bind
24663	3	7803	6	NULL	NULL	0	NULL	lipoproteins	NULL		induce	NULL				TF	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_163	12600889	31, 32 In contrast, the SRR mediates induction of TF expression by serum, lipoproteins, or shear stress 12, 13, 32 and contains three Sp1 and one Egr-1 binding sites.	bind
24664	4	7803	6	NULL	NULL	0	NULL	shear stress	NULL		induces	NULL				TF	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_163	12600889	31, 32 In contrast, the SRR mediates induction of TF expression by serum, lipoproteins, or shear stress 12, 13, 32 and contains three Sp1 and one Egr-1 binding sites.	bind
24665	5	7803	6	NULL	NULL	0	NULL		NULL		mediates	NULL			SRR	statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_163	12600889	31, 32 In contrast, the SRR mediates induction of TF expression by serum, lipoproteins, or shear stress 12, 13, 32 and contains three Sp1 and one Egr-1 binding sites.	bind
24666	6	7803	6	NULL	NULL	0	NULL		NULL		mediates	NULL			SRR	statement 4	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_163	12600889	31, 32 In contrast, the SRR mediates induction of TF expression by serum, lipoproteins, or shear stress 12, 13, 32 and contains three Sp1 and one Egr-1 binding sites.	bind
24667	7	7803	6	NULL	NULL	0	NULL		NULL		contains	NULL			SRR		NULL			Sp1 binding site	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_163	12600889	31, 32 In contrast, the SRR mediates induction of TF expression by serum, lipoproteins, or shear stress 12, 13, 32 and contains three Sp1 and one Egr-1 binding sites.	bind
24668	8	7803	6	NULL	NULL	0	NULL		NULL		contains	NULL			SRR		NULL			Egr-1 binding site	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_4_394_s_163	12600889	31, 32 In contrast, the SRR mediates induction of TF expression by serum, lipoproteins, or shear stress 12, 13, 32 and contains three Sp1 and one Egr-1 binding sites.	bind
31924	1	7804	5	13	NULL	NULL	NULL	5''-AMP	Chemical		bind					glycogen phosphorylase	GP	bovine;;liver			NULL		NULL	NULL	NULL	NULL	gw70_nature_439_7074_340_s_264	16421573	31, 57-64 (1982) |  PubMed |  ISI |  ChemPort |    arcia-Fuentes, L. ,  Camara-Artigas, A. ,  Lopez-Mayorga, [[ O.  &  Baron ]], C.   Thermodynamic characterization of 5''-AMP binding to bovine liver glycogen phosphorylase  a.  J. Biol. Chem. 271, 27569-27574 (1996) |  PubMed |  ChemPort |    aasik, [[ K.  &  Lee ]], C. C.  Reciprocal regulation of haem biosynthesis and the  circadian clock in mammals.	bind
24669	1	7804	6	10	NULL	0	NULL	5''-AMP	NULL		bind	NULL				 glycogen phosphorylase	NULL	bovine;;liver			NULL		NULL	NULL	NULL	NULL	gw70_nature_439_7074_340_s_264	16421573	31, 57-64 (1982) |  PubMed |  ISI |  ChemPort |    arcia-Fuentes, L. ,  Camara-Artigas, A. ,  Lopez-Mayorga, [[ O.  &  Baron ]], C.   Thermodynamic characterization of 5''-AMP binding to bovine liver glycogen phosphorylase  a.  J. Biol. Chem. 271, 27569-27574 (1996) |  PubMed |  ChemPort |    aasik, [[ K.  &  Lee ]], C. C.  Reciprocal regulation of haem biosynthesis and the  circadian clock in mammals.	bind
31925	1	7805	5	13	NULL	NULL	NULL	E2A	GP		mediates					p21Waf1/Cip1 gene	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_8333_s_124	14660614	31-kDa Represses E2A-mediated p21Waf1/Cip1 Gene Transcription by Inhibiting DNA Binding of E2A --	bind
31926	2	7805	5	13	NULL	NULL	NULL	E2A	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_8333_s_124	14660614	31-kDa Represses E2A-mediated p21Waf1/Cip1 Gene Transcription by Inhibiting DNA Binding of E2A --	bind
31927	3	7805	5	13	NULL	NULL	NULL	31-kDa protein	GP		inhibits					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_8333_s_124	14660614	31-kDa Represses E2A-mediated p21Waf1/Cip1 Gene Transcription by Inhibiting DNA Binding of E2A --	bind
31928	4	7805	5	13	NULL	NULL	NULL	statement 3	Process		represses					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_8333_s_124	14660614	31-kDa Represses E2A-mediated p21Waf1/Cip1 Gene Transcription by Inhibiting DNA Binding of E2A --	bind
38957	5	7805	5	13	NULL	NULL	NULL	statement 4	Process		causes					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_8333_s_124	14660614	31-kDa Represses E2A-mediated p21Waf1/Cip1 Gene Transcription by Inhibiting DNA Binding of E2A --	bind
24670	1	7805	6	NULL	NULL	0	NULL	E2A	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8333_s_124	14660614	31-kDa Represses E2A-mediated p21Waf1/Cip1 Gene Transcription by Inhibiting DNA Binding of E2A --	bind
24671	2	7805	6	NULL	NULL	0	NULL	E2A	NULL		mediates	NULL				p21Waf1/Cip1 Gene	NULL	transcription of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8333_s_124	14660614	31-kDa Represses E2A-mediated p21Waf1/Cip1 Gene Transcription by Inhibiting DNA Binding of E2A --	bind
24672	3	7805	6	NULL	NULL	0	NULL	31-kDa protein	NULL		represses	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_8333_s_124	14660614	31-kDa Represses E2A-mediated p21Waf1/Cip1 Gene Transcription by Inhibiting DNA Binding of E2A --	bind
24673	4	7805	6	10	NULL	0	NULL	statement 3			inhibits					statement 1					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_8333_s_124	14660614	31-kDa Represses E2A-mediated p21Waf1/Cip1 Gene Transcription by Inhibiting DNA Binding of E2A --	bind
24674	5	7805	6	NULL	NULL	0	NULL	statement 3	NULL		occurs by	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8333_s_124	14660614	31-kDa Represses E2A-mediated p21Waf1/Cip1 Gene Transcription by Inhibiting DNA Binding of E2A --	bind
31929	1	7807	5	13	NULL	NULL	NULL	PGA trianion	Chemical		bind					TIM	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_11_9544_s_47	12522213	31P NMR studies indicate that PGA binds to TIM as a trianion ( ).	bind
24676	1	7807	6	NULL	NULL	0	NULL	PGA 	NULL		bind	NULL				TIM	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_11_9544_s_47	12522213	31P NMR studies indicate that PGA binds to TIM as a trianion ( ).	bind
31930	1	7809	5	13	NULL	NULL	NULL	NADPH	Chemical		bind					dihydrofolate reductase	GP	 L. casei			NULL		NULL	NULL	NULL	NULL	gw60_structure_4_1_33_s_488	8805511	31P NMR studies of NADPH and NADP+ binding to  L. casei dihydrofolate reductase.	bind
31931	2	7809	5	13	NULL	NULL	NULL	NADP+	Chemical		bind					dihydrofolate reductase	GP	L. casei			NULL		NULL	NULL	NULL	NULL	gw60_structure_4_1_33_s_488	8805511	31P NMR studies of NADPH and NADP+ binding to  L. casei dihydrofolate reductase.	bind
24677	1	7809	6	NULL	NULL	0	NULL	NADPH	NULL		bind	NULL				dihydrofolate reductase	NULL	L.casei			NULL		0	NULL	NULL	NULL	gw60_structure_4_1_33_s_488	8805511	31P NMR studies of NADPH and NADP+ binding to  L. casei dihydrofolate reductase.	bind
24678	2	7809	6	NULL	NULL	0	NULL	NADP+	NULL		bind	NULL				dihydrofolate reductase	NULL	L.casei			NULL		0	NULL	NULL	NULL	gw60_structure_4_1_33_s_488	8805511	31P NMR studies of NADPH and NADP+ binding to  L. casei dihydrofolate reductase.	bind
31932	1	7810	5	13	NULL	NULL	NULL	d9	NucleicAcid		bind					XPA	GP		MBD		NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2635_s_211	11410673	31P resonances in the interior of d9 broadened and/or shifted before 31P resonances at the termini, suggesting that when d9 is bound to XPA-MBD the motion of the DNA is more restricted in the interior of the sequence than at the termini.	bind
31933	2	7810	5	13	NULL	NULL	NULL	statement 1	Process		restrict					DNA	NucleicAcid	motion of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2635_s_211	11410673	31P resonances in the interior of d9 broadened and/or shifted before 31P resonances at the termini, suggesting that when d9 is bound to XPA-MBD the motion of the DNA is more restricted in the interior of the sequence than at the termini.	bind
47123	3	7810	5	13	NULL	NULL	NULL	statement 2	Process		occurs upon					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2635_s_211	11410673	31P resonances in the interior of d9 broadened and/or shifted before 31P resonances at the termini, suggesting that when d9 is bound to XPA-MBD the motion of the DNA is more restricted in the interior of the sequence than at the termini.	bind
24679	1	7810	6	NULL	NULL	0	NULL	d9	NULL		bind	NULL				XPA	NULL		MBD		NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2635_s_211	11410673	31P resonances in the interior of d9 broadened and/or shifted before 31P resonances at the termini, suggesting that when d9 is bound to XPA-MBD the motion of the DNA is more restricted in the interior of the sequence than at the termini.	bind
24680	2	7810	6	10	NULL	0	NULL	statement 1	NULL		restrict	NULL				DNA	NULL	motion of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2635_s_211	11410673	31P resonances in the interior of d9 broadened and/or shifted before 31P resonances at the termini, suggesting that when d9 is bound to XPA-MBD the motion of the DNA is more restricted in the interior of the sequence than at the termini.	bind
24681	3	7810	6	10	NULL	0	NULL	statement 2	NULL		occurs upon	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2635_s_211	11410673	31P resonances in the interior of d9 broadened and/or shifted before 31P resonances at the termini, suggesting that when d9 is bound to XPA-MBD the motion of the DNA is more restricted in the interior of the sequence than at the termini.	bind
31934	1	7813	5	13	NULL	NULL	NULL	HVTs-SM1 cells	Cell	rapid;;continuous proliferation of	is associated with					SV40 LT antigen	Chemical	expression of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_3_636_s_205	10712385	32  Our results indicate that the rapid and continuous proliferation of HVTs-SM1 cells under permissive temperature conditions is associated with the expression of SV40 LT antigen and with LT-antigen binding and inactivation of p53.	bind
31935	2	7813	5	13	NULL	NULL	NULL	LT-antigen	Chemical		bind					p53	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_3_636_s_205	10712385	32  Our results indicate that the rapid and continuous proliferation of HVTs-SM1 cells under permissive temperature conditions is associated with the expression of SV40 LT antigen and with LT-antigen binding and inactivation of p53.	bind
31936	3	7813	5	13	NULL	NULL	NULL	statement 2	Process		inactivates					p53	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_3_636_s_205	10712385	32  Our results indicate that the rapid and continuous proliferation of HVTs-SM1 cells under permissive temperature conditions is associated with the expression of SV40 LT antigen and with LT-antigen binding and inactivation of p53.	bind
31937	4	7813	5	13	NULL	NULL	NULL	HVTs-SM1 cells	Cell	rapid;;continuous proliferation of	is associated with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_3_636_s_205	10712385	32  Our results indicate that the rapid and continuous proliferation of HVTs-SM1 cells under permissive temperature conditions is associated with the expression of SV40 LT antigen and with LT-antigen binding and inactivation of p53.	bind
31938	5	7813	5	13	NULL	NULL	NULL	HVTs-SM1 cells	Cell	rapid;;continuous proliferation of	is associated with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_3_636_s_205	10712385	32  Our results indicate that the rapid and continuous proliferation of HVTs-SM1 cells under permissive temperature conditions is associated with the expression of SV40 LT antigen and with LT-antigen binding and inactivation of p53.	bind
24907	1	7813	6	10	NULL	0	NULL	HVTs-SM1 cells	NULL	rapid;;continuous proliferation of	is associated with	NULL				SV40 LT antigen	NULL	expression of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_3_636_s_205	10712385	32  Our results indicate that the rapid and continuous proliferation of HVTs-SM1 cells under permissive temperature conditions is associated with the expression of SV40 LT antigen and with LT-antigen binding and inactivation of p53.	bind
24908	2	7813	6	NULL	NULL	0	NULL	LT-antigen	NULL		bind	NULL				p53	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_3_636_s_205	10712385	32  Our results indicate that the rapid and continuous proliferation of HVTs-SM1 cells under permissive temperature conditions is associated with the expression of SV40 LT antigen and with LT-antigen binding and inactivation of p53.	bind
24909	3	7813	6	10	NULL	0	NULL	statement 2			inactivates					p53					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_3_636_s_205	10712385	32  Our results indicate that the rapid and continuous proliferation of HVTs-SM1 cells under permissive temperature conditions is associated with the expression of SV40 LT antigen and with LT-antigen binding and inactivation of p53.	bind
24910	4	7813	6	10	NULL	0	NULL	HVTs-SM1 cells	NULL	rapid;;continuous proliferation of	is associated with	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_3_636_s_205	10712385	32  Our results indicate that the rapid and continuous proliferation of HVTs-SM1 cells under permissive temperature conditions is associated with the expression of SV40 LT antigen and with LT-antigen binding and inactivation of p53.	bind
24911	5	7813	6	10	NULL	0	NULL	HVTs-SM1 cells	NULL	rapid;;continuous proliferation of	is associated with	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_3_636_s_205	10712385	32  Our results indicate that the rapid and continuous proliferation of HVTs-SM1 cells under permissive temperature conditions is associated with the expression of SV40 LT antigen and with LT-antigen binding and inactivation of p53.	bind
31939	1	7815	5	13	NULL	NULL	NULL	IGTPase	GP		located in		predominantly			endoplasmic reticulum	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_6_704_s_243	10189358	32  Recent reports indicate that IGTPase is located predominantly in the endoplasmic reticulum of cells; however, GTP binding status of IGTPase is independent of its capacity to localize in the cellular compartment.	bind
31940	2	7815	5	13	NULL	NULL	NULL	IGTPase	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_6_704_s_243	10189358	32  Recent reports indicate that IGTPase is located predominantly in the endoplasmic reticulum of cells; however, GTP binding status of IGTPase is independent of its capacity to localize in the cellular compartment.	bind
31941	3	7815	5	13	NULL	NULL	NULL	statement 2	Process		is independent of					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_6_704_s_243	10189358	32  Recent reports indicate that IGTPase is located predominantly in the endoplasmic reticulum of cells; however, GTP binding status of IGTPase is independent of its capacity to localize in the cellular compartment.	bind
24682	1	7815	6	NULL	NULL	0	NULL	IGTPase	NULL		is located on	NULL	predominantly			endoplasmic reticulum	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_6_704_s_243	10189358	32  Recent reports indicate that IGTPase is located predominantly in the endoplasmic reticulum of cells; however, GTP binding status of IGTPase is independent of its capacity to localize in the cellular compartment.	bind
24683	2	7815	6	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				IGTPase	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_6_704_s_243	10189358	32  Recent reports indicate that IGTPase is located predominantly in the endoplasmic reticulum of cells; however, GTP binding status of IGTPase is independent of its capacity to localize in the cellular compartment.	bind
24684	3	7815	6	NULL	NULL	0	NULL	statement 2	NULL		is independent of	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_6_704_s_243	10189358	32  Recent reports indicate that IGTPase is located predominantly in the endoplasmic reticulum of cells; however, GTP binding status of IGTPase is independent of its capacity to localize in the cellular compartment.	bind
31942	1	7816	5	13	NULL	NULL	NULL	transcription factor	GP	nuclear	bind					AP-1/ets probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_8_1872_s_269	10446065	32  This result is consistent with our current observation (Figure 11  ) that anti - c-Jun and Jun-B antibodies blocked the binding of a nuclear transcription factor to the AP-1/ets probe.	bind
31943	2	7816	5	13	NULL	NULL	NULL	anti - c-Jun antibodies	GP		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_8_1872_s_269	10446065	32  This result is consistent with our current observation (Figure 11  ) that anti - c-Jun and Jun-B antibodies blocked the binding of a nuclear transcription factor to the AP-1/ets probe.	bind
31944	3	7816	5	13	NULL	NULL	NULL	anti - Jun-B antibodies	GP		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_8_1872_s_269	10446065	32  This result is consistent with our current observation (Figure 11  ) that anti - c-Jun and Jun-B antibodies blocked the binding of a nuclear transcription factor to the AP-1/ets probe.	bind
24685	1	7816	6	NULL	NULL	0	NULL	transcription factor	NULL	nuclear	bind	NULL				AP-1/ets probe	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_8_1872_s_269	10446065	32  This result is consistent with our current observation (Figure 11  ) that anti - c-Jun and Jun-B antibodies blocked the binding of a nuclear transcription factor to the AP-1/ets probe.	bind
24686	2	7816	6	NULL	NULL	0	NULL	anti - c-Jun antibody	NULL		blocks	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_8_1872_s_269	10446065	32  This result is consistent with our current observation (Figure 11  ) that anti - c-Jun and Jun-B antibodies blocked the binding of a nuclear transcription factor to the AP-1/ets probe.	bind
24687	3	7816	6	NULL	NULL	0	NULL	Jun-B antibody	NULL		blocks	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_8_1872_s_269	10446065	32  This result is consistent with our current observation (Figure 11  ) that anti - c-Jun and Jun-B antibodies blocked the binding of a nuclear transcription factor to the AP-1/ets probe.	bind
31945	1	7818	5	13	NULL	NULL	NULL	BTEB2	GP		bind									SE1	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_2_182_s_39	10417400	32  We demonstrate that basic transcriptional element (BTE) binding protein-2 (BTEB2) binds to the SE1 and regulates transcription of the SMemb gene.	bind
31946	2	7818	5	13	NULL	NULL	NULL	BTEB2	GP		is					basic transcriptional element binding protein-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_2_182_s_39	10417400	32  We demonstrate that basic transcriptional element (BTE) binding protein-2 (BTEB2) binds to the SE1 and regulates transcription of the SMemb gene.	bind
31947	3	7818	5	13	NULL	NULL	NULL	statement 1	Process		regulates					SMemb gene	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_2_182_s_39	10417400	32  We demonstrate that basic transcriptional element (BTE) binding protein-2 (BTEB2) binds to the SE1 and regulates transcription of the SMemb gene.	bind
24688	1	7818	6	NULL	NULL	0	NULL	BTEB2	NULL		bind	NULL				SE1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_85_2_182_s_39	10417400	32  We demonstrate that basic transcriptional element (BTE) binding protein-2 (BTEB2) binds to the SE1 and regulates transcription of the SMemb gene.	bind
24689	2	7818	6	NULL	NULL	0	NULL	BTEB-2	NULL		is	NULL				basic transcriptional element binding protein-2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_2_182_s_39	10417400	32  We demonstrate that basic transcriptional element (BTE) binding protein-2 (BTEB2) binds to the SE1 and regulates transcription of the SMemb gene.	bind
24691	3	7818	6	NULL	NULL	0	NULL	BTEB2	NULL		regulates	NULL				SMemb gene	NULL	transcription of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_2_182_s_39	10417400	32  We demonstrate that basic transcriptional element (BTE) binding protein-2 (BTEB2) binds to the SE1 and regulates transcription of the SMemb gene.	bind
31948	1	7819	5	13	NULL	NULL	NULL	Factor VII	GP		bind					TF	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_62	12231555	32 -  34 Factor VII binds to TF and is rapidly activated 35 by coagulation proteases 36 and by noncoagulation proteases, depending on the cellular location of the TF.	bind
31949	2	7819	5	13	NULL	NULL	NULL	coagulation proteases	GP		activates		rapidly			Factor VII	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_62	12231555	32 -  34 Factor VII binds to TF and is rapidly activated 35 by coagulation proteases 36 and by noncoagulation proteases, depending on the cellular location of the TF.	bind
31950	3	7819	5	13	NULL	NULL	NULL	noncoagulation proteases	GP		activates		rapidly			Factor VII	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_62	12231555	32 -  34 Factor VII binds to TF and is rapidly activated 35 by coagulation proteases 36 and by noncoagulation proteases, depending on the cellular location of the TF.	bind
31951	4	7819	5	13	NULL	NULL	NULL	statement 2	Process		is dependent on					TF	GP	cellular location of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_62	12231555	32 -  34 Factor VII binds to TF and is rapidly activated 35 by coagulation proteases 36 and by noncoagulation proteases, depending on the cellular location of the TF.	bind
31952	5	7819	5	13	NULL	NULL	NULL	statement 3	Process		is dependent on					TF	GP	cellular location of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_62	12231555	32 -  34 Factor VII binds to TF and is rapidly activated 35 by coagulation proteases 36 and by noncoagulation proteases, depending on the cellular location of the TF.	bind
24692	1	7819	6	NULL	NULL	0	NULL	factor VII	NULL		bind	NULL				TF	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_62	12231555	32 -  34 Factor VII binds to TF and is rapidly activated 35 by coagulation proteases 36 and by noncoagulation proteases, depending on the cellular location of the TF.	bind
24693	2	7819	6	10	NULL	0	NULL	coagulation proteases	NULL		activate	NULL	rapidly			factor VII	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_62	12231555	32 -  34 Factor VII binds to TF and is rapidly activated 35 by coagulation proteases 36 and by noncoagulation proteases, depending on the cellular location of the TF.	bind
24694	3	7819	6	10	NULL	0	NULL	noncoagulation proteases	NULL		activate	NULL	rapidly			factor VII	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_62	12231555	32 -  34 Factor VII binds to TF and is rapidly activated 35 by coagulation proteases 36 and by noncoagulation proteases, depending on the cellular location of the TF.	bind
38761	4	7819	6	NULL	NULL	0	NULL	statement 2	NULL		is dependent on	NULL				TF	NULL	cellular location of 			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_62	12231555	32 -  34 Factor VII binds to TF and is rapidly activated 35 by coagulation proteases 36 and by noncoagulation proteases, depending on the cellular location of the TF.	bind
38763	5	7819	6	NULL	NULL	0	NULL	statement 3	NULL		is dependent on	NULL				TF	NULL	cellular location of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_62	12231555	32 -  34 Factor VII binds to TF and is rapidly activated 35 by coagulation proteases 36 and by noncoagulation proteases, depending on the cellular location of the TF.	bind
31953	1	7820	5	13	NULL	NULL	NULL	uPAR	GP		colocalize with					cytokeratin-1	GP				NULL	endothelial cells	NULL	NULL	NULL	NULL	gw70_circulationres_94_9_1227_s_170	15044324	32 A recent study revealed that uPAR and cytokeratin-1 colocalize on endothelial cells and may form a receptor complex that mediates HK binding and the subsequent release of bradykinin.	bind
31954	2	7820	5	13	NULL	NULL	NULL	statement 1	Process		forms		may			receptor complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_9_1227_s_170	15044324	32 A recent study revealed that uPAR and cytokeratin-1 colocalize on endothelial cells and may form a receptor complex that mediates HK binding and the subsequent release of bradykinin.	bind
31955	3	7820	5	13	NULL	NULL	NULL	receptor complex	GP		mediates					HK	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_9_1227_s_170	15044324	32 A recent study revealed that uPAR and cytokeratin-1 colocalize on endothelial cells and may form a receptor complex that mediates HK binding and the subsequent release of bradykinin.	bind
31956	4	7820	5	13	NULL	NULL	NULL	statement 3	Process		mediates					bradykinin	GP	release of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_9_1227_s_170	15044324	32 A recent study revealed that uPAR and cytokeratin-1 colocalize on endothelial cells and may form a receptor complex that mediates HK binding and the subsequent release of bradykinin.	bind
24695	1	7820	6	NULL	NULL	0	NULL	uPAR	NULL		colocalize with	NULL				cytokeratin-1	NULL				NULL	endothelial cells	NULL	NULL	NULL	NULL	gw70_circulationres_94_9_1227_s_170	15044324	32 A recent study revealed that uPAR and cytokeratin-1 colocalize on endothelial cells and may form a receptor complex that mediates HK binding and the subsequent release of bradykinin.	bind
24697	2	7820	6	10	NULL	0	NULL	statement 1	NULL		form	NULL	may			receptor complex	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_9_1227_s_170	15044324	32 A recent study revealed that uPAR and cytokeratin-1 colocalize on endothelial cells and may form a receptor complex that mediates HK binding and the subsequent release of bradykinin.	bind
24698	3	7820	6	3	NULL	0	NULL	receptor complex	NULL		mediates	NULL				HK	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_9_1227_s_170	15044324	32 A recent study revealed that uPAR and cytokeratin-1 colocalize on endothelial cells and may form a receptor complex that mediates HK binding and the subsequent release of bradykinin.	bind
24699	4	7820	6	NULL	NULL	0	NULL	statement 3	NULL		mediates	NULL				bradykinin	NULL	release of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_9_1227_s_170	15044324	32 A recent study revealed that uPAR and cytokeratin-1 colocalize on endothelial cells and may form a receptor complex that mediates HK binding and the subsequent release of bradykinin.	bind
31957	1	7821	5	13	NULL	NULL	NULL	plasminogen	GP		bind					fibrin	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_6_1397_s_179	16574890	32 Because lysine residues in the fibrinogen molecule mediate the binding of plasminogen and tPA to fibrin, 38 lysine modification may impair plasminogen activation and fibrin cleavage by plasmin.	bind
31958	2	7821	5	13	NULL	NULL	NULL	tPA	GP		bind					fibrin	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_6_1397_s_179	16574890	32 Because lysine residues in the fibrinogen molecule mediate the binding of plasminogen and tPA to fibrin, 38 lysine modification may impair plasminogen activation and fibrin cleavage by plasmin.	bind
31959	3	7821	5	13	NULL	NULL	NULL	fibrinogen molecule	GP		mediates			lysine residues		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_6_1397_s_179	16574890	32 Because lysine residues in the fibrinogen molecule mediate the binding of plasminogen and tPA to fibrin, 38 lysine modification may impair plasminogen activation and fibrin cleavage by plasmin.	bind
31960	4	7821	5	13	NULL	NULL	NULL	fibrinogen molecule	GP		mediates			lysine residues		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_6_1397_s_179	16574890	32 Because lysine residues in the fibrinogen molecule mediate the binding of plasminogen and tPA to fibrin, 38 lysine modification may impair plasminogen activation and fibrin cleavage by plasmin.	bind
31961	5	7821	5	13	NULL	NULL	NULL	fibrinogen molecule	GP	modification of	impairs		may	lysine		plasminogen	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_6_1397_s_179	16574890	32 Because lysine residues in the fibrinogen molecule mediate the binding of plasminogen and tPA to fibrin, 38 lysine modification may impair plasminogen activation and fibrin cleavage by plasmin.	bind
31962	6	7821	5	13	NULL	NULL	NULL	plasmin	GP		cleaves					fibrin	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_6_1397_s_179	16574890	32 Because lysine residues in the fibrinogen molecule mediate the binding of plasminogen and tPA to fibrin, 38 lysine modification may impair plasminogen activation and fibrin cleavage by plasmin.	bind
31963	7	7821	5	13	NULL	NULL	NULL	fibrinogen molecule	GP	modification of	impairs		may	lysine		statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_6_1397_s_179	16574890	32 Because lysine residues in the fibrinogen molecule mediate the binding of plasminogen and tPA to fibrin, 38 lysine modification may impair plasminogen activation and fibrin cleavage by plasmin.	bind
24700	1	7821	6	NULL	NULL	0	NULL	plasminogen	NULL		bind	NULL				fibrin	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_6_1397_s_179	16574890	32 Because lysine residues in the fibrinogen molecule mediate the binding of plasminogen and tPA to fibrin, 38 lysine modification may impair plasminogen activation and fibrin cleavage by plasmin.	bind
24701	2	7821	6	NULL	NULL	0	NULL	tPA	NULL		bind	NULL				fibrin	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_6_1397_s_179	16574890	32 Because lysine residues in the fibrinogen molecule mediate the binding of plasminogen and tPA to fibrin, 38 lysine modification may impair plasminogen activation and fibrin cleavage by plasmin.	bind
24702	3	7821	6	NULL	NULL	0	NULL	fibrinogen molecule	NULL		mediate	NULL		lysine residues		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_6_1397_s_179	16574890	32 Because lysine residues in the fibrinogen molecule mediate the binding of plasminogen and tPA to fibrin, 38 lysine modification may impair plasminogen activation and fibrin cleavage by plasmin.	bind
24703	4	7821	6	NULL	NULL	0	NULL	fibrinogen molecule	NULL		mediate	NULL		lysine residues		statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_6_1397_s_179	16574890	32 Because lysine residues in the fibrinogen molecule mediate the binding of plasminogen and tPA to fibrin, 38 lysine modification may impair plasminogen activation and fibrin cleavage by plasmin.	bind
24704	5	7821	6	NULL	NULL	0	NULL	fibrinogen molecule	NULL	modification of	impair	NULL	may	lysine		plasminogen	NULL	activation of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_6_1397_s_179	16574890	32 Because lysine residues in the fibrinogen molecule mediate the binding of plasminogen and tPA to fibrin, 38 lysine modification may impair plasminogen activation and fibrin cleavage by plasmin.	bind
24705	6	7821	6	NULL	NULL	0	NULL	plasmin	NULL		cleaves	NULL				fibrin	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_6_1397_s_179	16574890	32 Because lysine residues in the fibrinogen molecule mediate the binding of plasminogen and tPA to fibrin, 38 lysine modification may impair plasminogen activation and fibrin cleavage by plasmin.	bind
24706	7	7821	6	NULL	NULL	0	NULL	fibrinogen molecule	NULL	modification of	impair	NULL	may	lysine residues		statement 6	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_6_1397_s_179	16574890	32 Because lysine residues in the fibrinogen molecule mediate the binding of plasminogen and tPA to fibrin, 38 lysine modification may impair plasminogen activation and fibrin cleavage by plasmin.	bind
31964	1	7822	5	13	NULL	NULL	NULL	VEGF-B	GP		bind					neuropilin 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_2_114_s_256	12805240	32 Binding of VEGF-B to neuropilin 1 might also mediate biological responses of VEGF-B.	bind
31965	2	7822	5	13	NULL	NULL	NULL	statement 1	Process		mediates					VEGF-B	GP	biological responses of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_2_114_s_256	12805240	32 Binding of VEGF-B to neuropilin 1 might also mediate biological responses of VEGF-B.	bind
24707	1	7822	6	NULL	NULL	0	NULL	VEGF-B	NULL		bind	NULL				neuropilin 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_93_2_114_s_256	12805240	32 Binding of VEGF-B to neuropilin 1 might also mediate biological responses of VEGF-B.	bind
24708	2	7822	6	NULL	NULL	0	NULL	statement 1	NULL		mediates	NULL	may			VEGF-B	NULL	biological responses of 			NULL		0	NULL	NULL	NULL	gw60_circulationres_93_2_114_s_256	12805240	32 Binding of VEGF-B to neuropilin 1 might also mediate biological responses of VEGF-B.	bind
31966	1	7823	5	13	NULL	NULL	NULL	SRF	GP		bind									CArG boxes	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_5_737_s_74	12740224	32 In addition to regulating growth-responsive genes such as c-fos, SRF binding to CArG boxes has been shown to regulate numerous muscle-specific genes.	bind
31967	2	7823	5	13	NULL	NULL	NULL	statement 1	Process		regulates					c-fos	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_5_737_s_74	12740224	32 In addition to regulating growth-responsive genes such as c-fos, SRF binding to CArG boxes has been shown to regulate numerous muscle-specific genes.	bind
31968	3	7823	5	13	NULL	NULL	NULL	c-fos	GP		is a type of					growth-responsive genes	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_5_737_s_74	12740224	32 In addition to regulating growth-responsive genes such as c-fos, SRF binding to CArG boxes has been shown to regulate numerous muscle-specific genes.	bind
31969	4	7823	5	13	NULL	NULL	NULL	statement 1	Process		regulates					muscle-specific genes	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_5_737_s_74	12740224	32 In addition to regulating growth-responsive genes such as c-fos, SRF binding to CArG boxes has been shown to regulate numerous muscle-specific genes.	bind
38960	5	7823	5	13	NULL	NULL	NULL	statement 1	Process		regulates					growth response genes	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_5_737_s_74	12740224	32 In addition to regulating growth-responsive genes such as c-fos, SRF binding to CArG boxes has been shown to regulate numerous muscle-specific genes.	bind
24709	1	7823	6	NULL	NULL	0	NULL	SRF	NULL		bind	NULL					NULL			CArG box	NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_5_737_s_74	12740224	32 In addition to regulating growth-responsive genes such as c-fos, SRF binding to CArG boxes has been shown to regulate numerous muscle-specific genes.	bind
24710	2	7823	6	NULL	NULL	0	NULL	statement 1	NULL		regulate	NULL				muscle specific genes	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_5_737_s_74	12740224	32 In addition to regulating growth-responsive genes such as c-fos, SRF binding to CArG boxes has been shown to regulate numerous muscle-specific genes.	bind
24711	3	7823	6	NULL	NULL	0	NULL	statement 1	NULL		regulates	NULL				growth responsive genes	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_5_737_s_74	12740224	32 In addition to regulating growth-responsive genes such as c-fos, SRF binding to CArG boxes has been shown to regulate numerous muscle-specific genes.	bind
38765	4	7823	6	NULL	NULL	0	NULL	c-fos	NULL		is a type of	NULL				growth responsive gene	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_5_737_s_74	12740224	32 In addition to regulating growth-responsive genes such as c-fos, SRF binding to CArG boxes has been shown to regulate numerous muscle-specific genes.	bind
38766	5	7823	6	NULL	NULL	0	NULL	statement 1	NULL		regulates	NULL				c-fos	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_5_737_s_74	12740224	32 In addition to regulating growth-responsive genes such as c-fos, SRF binding to CArG boxes has been shown to regulate numerous muscle-specific genes.	bind
31970	1	7824	5	13	NULL	NULL	NULL	p50-p65 heterodimer	GP		bind					I-kappaB	GP				NULL	cytosol of cells that have inducible NF-kappaB activity	NULL	NULL	NULL	NULL	gw60_circulation_98_21_2255_s_174	9826311	32 In cells that have inducible NF-kappaB activity, the factor comprises a p50-p65 heterodimer bound by an inhibitory subunit I-kappaB in the cytosol and can be activated by dissociation of I-kappaB.	bind
31971	2	7824	5	13	NULL	NULL	NULL	I-kappaB	GP	dissociation of	activates					p50-p65 heterodimer	GP				NULL	\tcytosol of cells that have inducible NF-kappaB activity	NULL	NULL	NULL	NULL	gw60_circulation_98_21_2255_s_174	9826311	32 In cells that have inducible NF-kappaB activity, the factor comprises a p50-p65 heterodimer bound by an inhibitory subunit I-kappaB in the cytosol and can be activated by dissociation of I-kappaB.	bind
31972	3	7824	5	13	NULL	NULL	NULL	I-kappaB	GP		is a type of					inhibitory subunit 	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_98_21_2255_s_174	9826311	32 In cells that have inducible NF-kappaB activity, the factor comprises a p50-p65 heterodimer bound by an inhibitory subunit I-kappaB in the cytosol and can be activated by dissociation of I-kappaB.	bind
24712	1	7824	6	10	NULL	0	NULL	p50-p65 heterodimer			bind					I-kappaB					NULL	\tcytosol of cells that have inducible NF-kappaB activity	NULL	NULL	NULL	NULL	gw60_circulation_98_21_2255_s_174	9826311	32 In cells that have inducible NF-kappaB activity, the factor comprises a p50-p65 heterodimer bound by an inhibitory subunit I-kappaB in the cytosol and can be activated by dissociation of I-kappaB.	bind
24713	2	7824	6	10	NULL	0	NULL	I-kappaB		dissociation of	activates					statement 1					NULL	\tcytosol of cells that have inducible NF-kappaB activity	NULL	NULL	NULL	NULL	gw60_circulation_98_21_2255_s_174	9826311	32 In cells that have inducible NF-kappaB activity, the factor comprises a p50-p65 heterodimer bound by an inhibitory subunit I-kappaB in the cytosol and can be activated by dissociation of I-kappaB.	bind
38767	3	7824	6	NULL	NULL	0	NULL	I-kappaB	NULL		is a type of	NULL				inhibitory subunit	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_98_21_2255_s_174	9826311	32 In cells that have inducible NF-kappaB activity, the factor comprises a p50-p65 heterodimer bound by an inhibitory subunit I-kappaB in the cytosol and can be activated by dissociation of I-kappaB.	bind
31973	1	7825	5	13	NULL	NULL	NULL	moesin	GP	phosphorylated;;human	bind			Thr558		ezrin	GP	phosphorylated	Thr567		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_181_s_70	14592842	32 Phosphorylation of the ezrin/radixin/moesin (ERM) substrates of Rho-kinase was measured, using a rabbit polyclonal antibody to phosphorylated human moesin (Thr558), which also binds to phosphorylated ezrin (Thr567) and radixin (Thr564).	bind
31974	2	7825	5	13	NULL	NULL	NULL	moesin	GP	phosphorylated;;human	bind			Thr558		radixin	GP	phosphorylated	Thr564		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_181_s_70	14592842	32 Phosphorylation of the ezrin/radixin/moesin (ERM) substrates of Rho-kinase was measured, using a rabbit polyclonal antibody to phosphorylated human moesin (Thr558), which also binds to phosphorylated ezrin (Thr567) and radixin (Thr564).	bind
38961	3	7825	5	13	NULL	NULL	NULL	ERM	GP		is					ezrin/radixin/moesin	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_181_s_70	14592842	32 Phosphorylation of the ezrin/radixin/moesin (ERM) substrates of Rho-kinase was measured, using a rabbit polyclonal antibody to phosphorylated human moesin (Thr558), which also binds to phosphorylated ezrin (Thr567) and radixin (Thr564).	bind
24714	1	7825	6	NULL	NULL	0	NULL	ERM	NULL		is	NULL				ezrin/radixin/moesin	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_181_s_70	14592842	32 Phosphorylation of the ezrin/radixin/moesin (ERM) substrates of Rho-kinase was measured, using a rabbit polyclonal antibody to phosphorylated human moesin (Thr558), which also binds to phosphorylated ezrin (Thr567) and radixin (Thr564).	bind
24715	2	7825	6	10	NULL	0	NULL	moesin		human;;phosphorylated	bind			Thr558		ezrin		phosphorylated	Thr567		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_181_s_70	14592842	32 Phosphorylation of the ezrin/radixin/moesin (ERM) substrates of Rho-kinase was measured, using a rabbit polyclonal antibody to phosphorylated human moesin (Thr558), which also binds to phosphorylated ezrin (Thr567) and radixin (Thr564).	bind
24716	3	7825	6	10	NULL	0	NULL	moesin		phosphorylated;;human	bind					radixin		phosphorylated	Thr564		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_181_s_70	14592842	32 Phosphorylation of the ezrin/radixin/moesin (ERM) substrates of Rho-kinase was measured, using a rabbit polyclonal antibody to phosphorylated human moesin (Thr558), which also binds to phosphorylated ezrin (Thr567) and radixin (Thr564).	bind
31975	1	7826	5	13	NULL	NULL	NULL	LPS	Chemical		express					inflammatory mediators	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_3_236_s_236	16002747	32 Similarly, anti-CD14 antibodies inhibit the expression of inflammatory mediators by LPS. 25 In the current study, we found that L-4F prevented the binding of LPS to LBP in a concentration-dependent manner.	bind
31976	2	7826	5	13	NULL	NULL	NULL	anti-CD14 antibodies	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_3_236_s_236	16002747	32 Similarly, anti-CD14 antibodies inhibit the expression of inflammatory mediators by LPS. 25 In the current study, we found that L-4F prevented the binding of LPS to LBP in a concentration-dependent manner.	bind
31977	3	7826	5	13	NULL	NULL	NULL	LPS	Chemical		bind					LBP	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_3_236_s_236	16002747	32 Similarly, anti-CD14 antibodies inhibit the expression of inflammatory mediators by LPS. 25 In the current study, we found that L-4F prevented the binding of LPS to LBP in a concentration-dependent manner.	bind
31978	4	7826	5	13	NULL	NULL	NULL	L-4F	GP		prevents					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_3_236_s_236	16002747	32 Similarly, anti-CD14 antibodies inhibit the expression of inflammatory mediators by LPS. 25 In the current study, we found that L-4F prevented the binding of LPS to LBP in a concentration-dependent manner.	bind
31979	5	7826	5	13	NULL	NULL	NULL	statement 4	Process		is dependent on					concentration					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_3_236_s_236	16002747	32 Similarly, anti-CD14 antibodies inhibit the expression of inflammatory mediators by LPS. 25 In the current study, we found that L-4F prevented the binding of LPS to LBP in a concentration-dependent manner.	bind
24717	1	7826	6	NULL	NULL	0	NULL	LPS	NULL		bind	NULL				LBP	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_3_236_s_236	16002747	32 Similarly, anti-CD14 antibodies inhibit the expression of inflammatory mediators by LPS. 25 In the current study, we found that L-4F prevented the binding of LPS to LBP in a concentration-dependent manner.	bind
24718	2	7826	6	NULL	NULL	0	NULL	L-4F	NULL		prevents	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_3_236_s_236	16002747	32 Similarly, anti-CD14 antibodies inhibit the expression of inflammatory mediators by LPS. 25 In the current study, we found that L-4F prevented the binding of LPS to LBP in a concentration-dependent manner.	bind
24719	3	7826	6	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				concentration	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_3_236_s_236	16002747	32 Similarly, anti-CD14 antibodies inhibit the expression of inflammatory mediators by LPS. 25 In the current study, we found that L-4F prevented the binding of LPS to LBP in a concentration-dependent manner.	bind
24721	5	7826	6	10	NULL	0	NULL	anti-CD14 antibodies			inhibits					statement 4					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_3_236_s_236	16002747	32 Similarly, anti-CD14 antibodies inhibit the expression of inflammatory mediators by LPS. 25 In the current study, we found that L-4F prevented the binding of LPS to LBP in a concentration-dependent manner.	bind
24740	4	7826	6	10	NULL	0	NULL	LPS			express					\tinflammatory mediators					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_3_236_s_236	16002747	32 Similarly, anti-CD14 antibodies inhibit the expression of inflammatory mediators by LPS. 25 In the current study, we found that L-4F prevented the binding of LPS to LBP in a concentration-dependent manner.	bind
31980	1	7827	5	13	NULL	NULL	NULL	p27Kip1	GP		inhibits					cdk	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_4_1129_s_150	10514396	32 The mechanism by which p27Kip1 inhibits cdk activity is not fully understood, but it appears that binding of p27Kip1 to the cyclin D2/cdk4 complex sequesters the inhibitor away from the cyclin E/cdk2 complex, causing inactivation of the latter.	bind
31981	2	7827	5	13	NULL	NULL	NULL	p27Kip1	GP		bind					cyclin D2/cdk4 complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_4_1129_s_150	10514396	32 The mechanism by which p27Kip1 inhibits cdk activity is not fully understood, but it appears that binding of p27Kip1 to the cyclin D2/cdk4 complex sequesters the inhibitor away from the cyclin E/cdk2 complex, causing inactivation of the latter.	bind
31982	3	7827	5	13	NULL	NULL	NULL	p27Kip1	GP		sequestered from					cyclin E/cdk2 complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_4_1129_s_150	10514396	32 The mechanism by which p27Kip1 inhibits cdk activity is not fully understood, but it appears that binding of p27Kip1 to the cyclin D2/cdk4 complex sequesters the inhibitor away from the cyclin E/cdk2 complex, causing inactivation of the latter.	bind
31983	4	7827	5	13	NULL	NULL	NULL	statement 2	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_4_1129_s_150	10514396	32 The mechanism by which p27Kip1 inhibits cdk activity is not fully understood, but it appears that binding of p27Kip1 to the cyclin D2/cdk4 complex sequesters the inhibitor away from the cyclin E/cdk2 complex, causing inactivation of the latter.	bind
31984	5	7827	5	13	NULL	NULL	NULL	statement 3	Process		inactivates					cyclin E/cdk2 complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_4_1129_s_150	10514396	32 The mechanism by which p27Kip1 inhibits cdk activity is not fully understood, but it appears that binding of p27Kip1 to the cyclin D2/cdk4 complex sequesters the inhibitor away from the cyclin E/cdk2 complex, causing inactivation of the latter.	bind
24741	1	7827	6	NULL	NULL	0	NULL	p27Kip1	NULL		bind	NULL				cyclin D2/cdk4 complex	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_4_1129_s_150	10514396	32 The mechanism by which p27Kip1 inhibits cdk activity is not fully understood, but it appears that binding of p27Kip1 to the cyclin D2/cdk4 complex sequesters the inhibitor away from the cyclin E/cdk2 complex, causing inactivation of the latter.	bind
24912	2	7827	6	NULL	NULL	0	NULL	statement 1	NULL		sequesters	NULL				p27Kip1 	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_4_1129_s_150	10514396	32 The mechanism by which p27Kip1 inhibits cdk activity is not fully understood, but it appears that binding of p27Kip1 to the cyclin D2/cdk4 complex sequesters the inhibitor away from the cyclin E/cdk2 complex, causing inactivation of the latter.	bind
24913	3	7827	6	NULL	NULL	0	NULL	p27kip1	NULL		is sequestered from	NULL				cyclin E/cdk2 complex	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_4_1129_s_150	10514396	32 The mechanism by which p27Kip1 inhibits cdk activity is not fully understood, but it appears that binding of p27Kip1 to the cyclin D2/cdk4 complex sequesters the inhibitor away from the cyclin E/cdk2 complex, causing inactivation of the latter.	bind
24914	4	7827	6	NULL	NULL	0	NULL	statement 2	NULL		inactivates	NULL				cyclin E/cdk2 complex	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_4_1129_s_150	10514396	32 The mechanism by which p27Kip1 inhibits cdk activity is not fully understood, but it appears that binding of p27Kip1 to the cyclin D2/cdk4 complex sequesters the inhibitor away from the cyclin E/cdk2 complex, causing inactivation of the latter.	bind
25133	5	7827	6	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_4_1129_s_150	10514396	32 The mechanism by which p27Kip1 inhibits cdk activity is not fully understood, but it appears that binding of p27Kip1 to the cyclin D2/cdk4 complex sequesters the inhibitor away from the cyclin E/cdk2 complex, causing inactivation of the latter.	bind
31985	1	7828	5	13	NULL	NULL	NULL	ephrin-B1	GP		bind					Grb4	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_2_190_s_224	12588758	32 The observation that the region of ephrin-B1 binding to Grb4 is conserved in ephrin-B2 cytoplasmic tail suggests that EphB4 reverse signaling through ephrin-B2 may be similar through EphB2 reverse signaling through ephrin-B1.	bind
31986	2	7828	5	13	NULL	NULL	NULL	statement 1	Process	region of	is conserved in					ephrin-B2	GP		cytoplasmic tail		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_2_190_s_224	12588758	32 The observation that the region of ephrin-B1 binding to Grb4 is conserved in ephrin-B2 cytoplasmic tail suggests that EphB4 reverse signaling through ephrin-B2 may be similar through EphB2 reverse signaling through ephrin-B1.	bind
31987	3	7828	5	13	NULL	NULL	NULL	EphB4	GP		reverse signal through					ephrin-B2	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_2_190_s_224	12588758	32 The observation that the region of ephrin-B1 binding to Grb4 is conserved in ephrin-B2 cytoplasmic tail suggests that EphB4 reverse signaling through ephrin-B2 may be similar through EphB2 reverse signaling through ephrin-B1.	bind
31988	4	7828	5	13	NULL	NULL	NULL	EphB2	GP		reverse signal through					ephrin-B1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_2_190_s_224	12588758	32 The observation that the region of ephrin-B1 binding to Grb4 is conserved in ephrin-B2 cytoplasmic tail suggests that EphB4 reverse signaling through ephrin-B2 may be similar through EphB2 reverse signaling through ephrin-B1.	bind
31989	5	7828	5	13	NULL	NULL	NULL	statement 3	Process		similar to		may			statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_2_190_s_224	12588758	32 The observation that the region of ephrin-B1 binding to Grb4 is conserved in ephrin-B2 cytoplasmic tail suggests that EphB4 reverse signaling through ephrin-B2 may be similar through EphB2 reverse signaling through ephrin-B1.	bind
24742	1	7828	6	NULL	NULL	0	NULL	ephrin-B1	NULL		bind	NULL				Grb4	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_2_190_s_224	12588758	32 The observation that the region of ephrin-B1 binding to Grb4 is conserved in ephrin-B2 cytoplasmic tail suggests that EphB4 reverse signaling through ephrin-B2 may be similar through EphB2 reverse signaling through ephrin-B1.	bind
24915	2	7828	6	NULL	NULL	0	NULL	EphB4	NULL		reverse signals through	NULL				ephrin-B2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_2_190_s_224	12588758	32 The observation that the region of ephrin-B1 binding to Grb4 is conserved in ephrin-B2 cytoplasmic tail suggests that EphB4 reverse signaling through ephrin-B2 may be similar through EphB2 reverse signaling through ephrin-B1.	bind
24916	3	7828	6	NULL	NULL	0	NULL	EphB2	NULL		reverse signals through	NULL				ephrin-B1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_2_190_s_224	12588758	32 The observation that the region of ephrin-B1 binding to Grb4 is conserved in ephrin-B2 cytoplasmic tail suggests that EphB4 reverse signaling through ephrin-B2 may be similar through EphB2 reverse signaling through ephrin-B1.	bind
24917	4	7828	6	10	NULL	0	NULL	statement 2	NULL		 similar to	NULL	may be			statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_2_190_s_224	12588758	32 The observation that the region of ephrin-B1 binding to Grb4 is conserved in ephrin-B2 cytoplasmic tail suggests that EphB4 reverse signaling through ephrin-B2 may be similar through EphB2 reverse signaling through ephrin-B1.	bind
38768	5	7828	6	NULL	NULL	0	NULL	statement 1	NULL	region of	is conserved in	NULL				ephrin-B2	NULL		cytoplasmic tail		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_2_190_s_224	12588758	32 The observation that the region of ephrin-B1 binding to Grb4 is conserved in ephrin-B2 cytoplasmic tail suggests that EphB4 reverse signaling through ephrin-B2 may be similar through EphB2 reverse signaling through ephrin-B1.	bind
31990	1	7829	5	13	NULL	NULL	NULL	TnI	GP		bind					TnC	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_89_12_1184_s_160	11739284	32, 33 Because the interaction between TnI and TnC increases Ca2+ binding, reduced TnI/TnC binding lowers the affinity of TnC for Ca2+.	bind
31991	2	7829	5	13	NULL	NULL	NULL	statement 1	Process		increases					Ca2+	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_89_12_1184_s_160	11739284	32, 33 Because the interaction between TnI and TnC increases Ca2+ binding, reduced TnI/TnC binding lowers the affinity of TnC for Ca2+.	bind
31992	3	7829	5	13	NULL	NULL	NULL	TnC	GP		bind					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_89_12_1184_s_160	11739284	32, 33 Because the interaction between TnI and TnC increases Ca2+ binding, reduced TnI/TnC binding lowers the affinity of TnC for Ca2+.	bind
31993	4	7829	5	13	NULL	NULL	NULL	statement 1	Process	reduced	lowers					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_89_12_1184_s_160	11739284	32, 33 Because the interaction between TnI and TnC increases Ca2+ binding, reduced TnI/TnC binding lowers the affinity of TnC for Ca2+.	bind
24743	1	7829	6	NULL	NULL	0	NULL	TnI	NULL		interacts with	NULL				TnC	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_89_12_1184_s_160	11739284	32, 33 Because the interaction between TnI and TnC increases Ca2+ binding, reduced TnI/TnC binding lowers the affinity of TnC for Ca2+.	bind
24744	2	7829	6	NULL	NULL	0	NULL	statement 1	NULL		increases	NULL				Ca2+	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_circulationres_89_12_1184_s_160	11739284	32, 33 Because the interaction between TnI and TnC increases Ca2+ binding, reduced TnI/TnC binding lowers the affinity of TnC for Ca2+.	bind
24745	3	7829	6	NULL	NULL	0	NULL	TnC	NULL		has affinity for	NULL				Ca2+	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_89_12_1184_s_160	11739284	32, 33 Because the interaction between TnI and TnC increases Ca2+ binding, reduced TnI/TnC binding lowers the affinity of TnC for Ca2+.	bind
24746	4	7829	6	NULL	NULL	0	NULL	statement 1	NULL	reduced	lowers	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_89_12_1184_s_160	11739284	32, 33 Because the interaction between TnI and TnC increases Ca2+ binding, reduced TnI/TnC binding lowers the affinity of TnC for Ca2+.	bind
31994	1	7830	5	13	NULL	NULL	NULL	RANTES	GP		bind					CCR5	GP				NULL	T cells	NULL	NULL	NULL	NULL	gw60_amjpathol_162_5_1591_s_124	12707043	32,33 For function-blocking studies, the binding of RANTES to CCR5 on the T cells was neutralized by preincubating the T cells with an anti-CCR5 monoclonal antibody (20 mug/ml final concentration) for 15 minutes on ice.	bind
24747	1	7830	6	NULL	NULL	0	NULL	RANTES	NULL		bind	NULL				CCR5	NULL				NULL	T cells	0	NULL	NULL	NULL	gw60_amjpathol_162_5_1591_s_124	12707043	32,33 For function-blocking studies, the binding of RANTES to CCR5 on the T cells was neutralized by preincubating the T cells with an anti-CCR5 monoclonal antibody (20 mug/ml final concentration) for 15 minutes on ice.	bind
31995	1	7831	5	13	NULL	NULL	NULL	HDL core	GP		becomes rich in					triglyceride	Chemical				NULL	hypertriglyceridemia	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3021_s_224	9409289	32,52,54 In hypertriglyceridemia, the core of HDL may become rich in triglyceride whereby subsequent lipolysis of HDL core by hepatic lipase may loosen the binding of apoA-I to HDL particle and facilitate clearance of apoA-I by the kidneys.	bind
31996	2	7831	5	13	NULL	NULL	NULL	lipase	GP	hepatic	lipolyse					HDL core	GP				NULL	hypertriglyceridemia	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3021_s_224	9409289	32,52,54 In hypertriglyceridemia, the core of HDL may become rich in triglyceride whereby subsequent lipolysis of HDL core by hepatic lipase may loosen the binding of apoA-I to HDL particle and facilitate clearance of apoA-I by the kidneys.	bind
31997	3	7831	5	13	NULL	NULL	NULL	apoA-I	GP		bind					HDL particle	GP				NULL	hypertriglyceridemia	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3021_s_224	9409289	32,52,54 In hypertriglyceridemia, the core of HDL may become rich in triglyceride whereby subsequent lipolysis of HDL core by hepatic lipase may loosen the binding of apoA-I to HDL particle and facilitate clearance of apoA-I by the kidneys.	bind
31998	4	7831	5	13	NULL	NULL	NULL	statement 2	Process		loosen		may			statement 3	Process				NULL	hypertriglyceridemia	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3021_s_224	9409289	32,52,54 In hypertriglyceridemia, the core of HDL may become rich in triglyceride whereby subsequent lipolysis of HDL core by hepatic lipase may loosen the binding of apoA-I to HDL particle and facilitate clearance of apoA-I by the kidneys.	bind
31999	5	7831	5	13	NULL	NULL	NULL	apoA-I 	GP		cleared by					kidneys	OrganismPart				NULL	hypertriglyceridemia	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3021_s_224	9409289	32,52,54 In hypertriglyceridemia, the core of HDL may become rich in triglyceride whereby subsequent lipolysis of HDL core by hepatic lipase may loosen the binding of apoA-I to HDL particle and facilitate clearance of apoA-I by the kidneys.	bind
32000	6	7831	5	13	NULL	NULL	NULL	statement 2	Process		facilitate					statement 5	Process				NULL	hypertriglyceridemia	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3021_s_224	9409289	32,52,54 In hypertriglyceridemia, the core of HDL may become rich in triglyceride whereby subsequent lipolysis of HDL core by hepatic lipase may loosen the binding of apoA-I to HDL particle and facilitate clearance of apoA-I by the kidneys.	bind
24748	1	7831	6	NULL	NULL	0	NULL	apoA-I	NULL		bind	NULL				HDL particle	NULL				NULL	hypertriglyceridemia	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3021_s_224	9409289	32,52,54 In hypertriglyceridemia, the core of HDL may become rich in triglyceride whereby subsequent lipolysis of HDL core by hepatic lipase may loosen the binding of apoA-I to HDL particle and facilitate clearance of apoA-I by the kidneys.	bind
24918	2	7831	6	NULL	NULL	0	NULL	HDL core 	NULL		becomes rich in	NULL				triglyceride	NULL				NULL	hypertriglyceridemia	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3021_s_224	9409289	32,52,54 In hypertriglyceridemia, the core of HDL may become rich in triglyceride whereby subsequent lipolysis of HDL core by hepatic lipase may loosen the binding of apoA-I to HDL particle and facilitate clearance of apoA-I by the kidneys.	bind
24919	3	7831	6	10	NULL	0	NULL	apoA-I			cleared by					kidney					NULL	hypertriglyceridemia	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3021_s_224	9409289	32,52,54 In hypertriglyceridemia, the core of HDL may become rich in triglyceride whereby subsequent lipolysis of HDL core by hepatic lipase may loosen the binding of apoA-I to HDL particle and facilitate clearance of apoA-I by the kidneys.	bind
24920	4	7831	6	NULL	NULL	0	NULL	hepatic lipase	NULL		lipolyse	NULL				HDL core	NULL				NULL	hypertriglyceridemia	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3021_s_224	9409289	32,52,54 In hypertriglyceridemia, the core of HDL may become rich in triglyceride whereby subsequent lipolysis of HDL core by hepatic lipase may loosen the binding of apoA-I to HDL particle and facilitate clearance of apoA-I by the kidneys.	bind
24921	5	7831	6	NULL	NULL	0	NULL	statement 4	NULL		loosen	NULL	may			statement 1	NULL				NULL	hypertriglyceridemia	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3021_s_224	9409289	32,52,54 In hypertriglyceridemia, the core of HDL may become rich in triglyceride whereby subsequent lipolysis of HDL core by hepatic lipase may loosen the binding of apoA-I to HDL particle and facilitate clearance of apoA-I by the kidneys.	bind
24922	6	7831	6	10	NULL	0	NULL	statement 4			facilitate					statement 3					NULL	hypertriglyceridemia	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3021_s_224	9409289	32,52,54 In hypertriglyceridemia, the core of HDL may become rich in triglyceride whereby subsequent lipolysis of HDL core by hepatic lipase may loosen the binding of apoA-I to HDL particle and facilitate clearance of apoA-I by the kidneys.	bind
32001	1	7833	5	13	NULL	NULL	NULL	p47phox species	GP		bind					TRAF4	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_6_2320_s_154	15743827	32P labeling to assess the nature of the p47phox species bound to TRAF4.	bind
24749	1	7833	6	NULL	NULL	0	NULL	p47phox species	NULL		bind	NULL				TRAF4	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_6_2320_s_154	15743827	32P labeling to assess the nature of the p47phox species bound to TRAF4.	bind
32002	1	7834	5	13	NULL	NULL	NULL	Ku70/86	GP	purified;;native	bind					PARP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_29_20521_s_219	10400681	32P-End-labeled DNA fragments were circularized by blunt end ligation, and the binding of column purified native Ku70/86 and PARP was analyzed by EMSA as described under	bind
24751	1	7834	6	10	NULL	0	NULL	Ku70/86	NULL	purified;; native	bind	NULL				PARP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_29_20521_s_219	10400681	32P-End-labeled DNA fragments were circularized by blunt end ligation, and the binding of column purified native Ku70/86 and PARP was analyzed by EMSA as described under	bind
32003	1	7835	5	13	NULL	NULL	NULL	GST-Yra1p	GP		bind					Mex67p/Mtr2p	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_3_410_s_142	10722314	32P-labeled  SSA1 RNA (bp 818-1152) was incubated with GST, GST-Yra1p on beads, and GST-Yra1p bound to Mex67p/Mtr2p on beads.	bind
24764	1	7835	6	NULL	NULL	0	NULL	GST-Yra1p	NULL		bind	NULL				Mex67p/Mtr2p	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_19_3_410_s_142	10722314	32P-labeled  SSA1 RNA (bp 818-1152) was incubated with GST, GST-Yra1p on beads, and GST-Yra1p bound to Mex67p/Mtr2p on beads.	bind
32004	1	7836	5	13	NULL	NULL	NULL	5ABC	GP	32P-labeled	bind					GST-MSP142	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_9_5164_s_159	12692305	32P-labeled 5ABC (10, 20, 40, and 80 muM) and 5BC (21, 42, 84, and 168 muM) bound to GST-MSP142	bind
32005	2	7836	5	13	NULL	NULL	NULL	5BC	GP	32P-labeled	bind					GST-MSP142	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_9_5164_s_159	12692305	32P-labeled 5ABC (10, 20, 40, and 80 muM) and 5BC (21, 42, 84, and 168 muM) bound to GST-MSP142	bind
24779	1	7836	6	10	NULL	0	NULL	5ABC		32P-labeled 	bind					GST-MSP142					NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_9_5164_s_159	12692305	32P-labeled 5ABC (10, 20, 40, and 80 muM) and 5BC (21, 42, 84, and 168 muM) bound to GST-MSP142	bind
24780	2	7836	6	10	NULL	0	NULL	5BC		32P-labeled 	bind					GST-MSP142					NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_9_5164_s_159	12692305	32P-labeled 5ABC (10, 20, 40, and 80 muM) and 5BC (21, 42, 84, and 168 muM) bound to GST-MSP142	bind
32006	1	7837	5	13	NULL	NULL	NULL	guanidine nucleotides	Chemical	 labeled	bind					Rap1	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_278_5335_124_s_96	9311917	32P-labeled anergic or control cells (2 x 107 cells per sample) were unstimulated ( ) or stimulated (+) ( 33) for 5 min. Labeled guanidine nucleotides bound to Rap1 or Ras were quantitated, and results were expressed as percent of GTP bound to Rap1 or Ras proteins relative to the total amount of guanidine nucleotides (GTP+GDP) complexed to these proteins.	bind
32007	2	7837	5	13	NULL	NULL	NULL	guanidine nucleotides	Chemical	labeled	bind					Ras	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_278_5335_124_s_96	9311917	32P-labeled anergic or control cells (2 x 107 cells per sample) were unstimulated ( ) or stimulated (+) ( 33) for 5 min. Labeled guanidine nucleotides bound to Rap1 or Ras were quantitated, and results were expressed as percent of GTP bound to Rap1 or Ras proteins relative to the total amount of guanidine nucleotides (GTP+GDP) complexed to these proteins.	bind
32008	3	7837	5	13	NULL	NULL	NULL	statement 1	Process		is alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_278_5335_124_s_96	9311917	32P-labeled anergic or control cells (2 x 107 cells per sample) were unstimulated ( ) or stimulated (+) ( 33) for 5 min. Labeled guanidine nucleotides bound to Rap1 or Ras were quantitated, and results were expressed as percent of GTP bound to Rap1 or Ras proteins relative to the total amount of guanidine nucleotides (GTP+GDP) complexed to these proteins.	bind
55551	4	7837	5	13	NULL	NULL	NULL	guanidine nucleotides	Chemical		is					GTP+GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_278_5335_124_s_96	9311917	32P-labeled anergic or control cells (2 x 107 cells per sample) were unstimulated ( ) or stimulated (+) ( 33) for 5 min. Labeled guanidine nucleotides bound to Rap1 or Ras were quantitated, and results were expressed as percent of GTP bound to Rap1 or Ras proteins relative to the total amount of guanidine nucleotides (GTP+GDP) complexed to these proteins.	bind
24923	1	7837	6	NULL	NULL	0	NULL	guanidine nucleotides	NULL	labeled	bind	NULL				Rap1	NULL				NULL		0	NULL	NULL	NULL	gw60_science_278_5335_124_s_96	9311917	32P-labeled anergic or control cells (2 x 107 cells per sample) were unstimulated ( ) or stimulated (+) ( 33) for 5 min. Labeled guanidine nucleotides bound to Rap1 or Ras were quantitated, and results were expressed as percent of GTP bound to Rap1 or Ras proteins relative to the total amount of guanidine nucleotides (GTP+GDP) complexed to these proteins.	bind
24924	2	7837	6	NULL	NULL	0	NULL	guanidine nucleotides	NULL	labeled	bind	NULL				Ras	NULL				NULL		0	NULL	NULL	NULL	gw60_science_278_5335_124_s_96	9311917	32P-labeled anergic or control cells (2 x 107 cells per sample) were unstimulated ( ) or stimulated (+) ( 33) for 5 min. Labeled guanidine nucleotides bound to Rap1 or Ras were quantitated, and results were expressed as percent of GTP bound to Rap1 or Ras proteins relative to the total amount of guanidine nucleotides (GTP+GDP) complexed to these proteins.	bind
25134	3	7837	6	10	NULL	0	NULL	guanidine nucleotides			is					GTP+GDP					NULL		NULL	NULL	NULL	NULL	gw60_science_278_5335_124_s_96	9311917	32P-labeled anergic or control cells (2 x 107 cells per sample) were unstimulated ( ) or stimulated (+) ( 33) for 5 min. Labeled guanidine nucleotides bound to Rap1 or Ras were quantitated, and results were expressed as percent of GTP bound to Rap1 or Ras proteins relative to the total amount of guanidine nucleotides (GTP+GDP) complexed to these proteins.	bind
47358	4	7837	6	10	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_science_278_5335_124_s_96	9311917	32P-labeled anergic or control cells (2 x 107 cells per sample) were unstimulated ( ) or stimulated (+) ( 33) for 5 min. Labeled guanidine nucleotides bound to Rap1 or Ras were quantitated, and results were expressed as percent of GTP bound to Rap1 or Ras proteins relative to the total amount of guanidine nucleotides (GTP+GDP) complexed to these proteins.	bind
32009	1	7838	5	13	NULL	NULL	NULL	GST-N-Shh	GP	32P-Labeled	bind					megalin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25660_s_148	11964399	32P-Labeled GST-N-Shh bound to megalin, and the binding was inhibited in a dose-dependent manner by the addition of unlabeled GST-N-Shh (Fig.  4 B).	bind
32010	2	7838	5	13	NULL	NULL	NULL	GST-N-Shh	GP	unlabeled	inhibits		dose dependent			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25660_s_148	11964399	32P-Labeled GST-N-Shh bound to megalin, and the binding was inhibited in a dose-dependent manner by the addition of unlabeled GST-N-Shh (Fig.  4 B).	bind
24783	1	7838	6	10	NULL	0	NULL	GST-N-Shh	NULL	32P-Labeled 	bind	NULL				megalin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_28_25660_s_148	11964399	32P-Labeled GST-N-Shh bound to megalin, and the binding was inhibited in a dose-dependent manner by the addition of unlabeled GST-N-Shh (Fig.  4 B).	bind
24785	2	7838	6	NULL	NULL	0	NULL	GST-N-Shh	NULL	unlabeled	inhibits	NULL	dose dependently			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_28_25660_s_148	11964399	32P-Labeled GST-N-Shh bound to megalin, and the binding was inhibited in a dose-dependent manner by the addition of unlabeled GST-N-Shh (Fig.  4 B).	bind
32011	1	7841	5	13	NULL	NULL	NULL	nicotinamide adenine dinucleotide	Chemical	folded conformation of	bind					flavin reductase	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_21_4294_s_544	11691917	33       Tanner,J.J., Tu,S.C., Barbour,L.J., Barnes,C.L. and Krause,K.L. (1999) Unusual folded conformation of nicotinamide adenine dinucleotide bound to flavin reductase P.  Protein Sci.,  8, 1725 - 1732.	bind
24787	1	7841	6	NULL	NULL	0	NULL	nicotinamide adenine dinucleotide	NULL	folded conformation of 	bind	NULL				flavin reductase	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_21_4294_s_544	11691917	33       Tanner,J.J., Tu,S.C., Barbour,L.J., Barnes,C.L. and Krause,K.L. (1999) Unusual folded conformation of nicotinamide adenine dinucleotide bound to flavin reductase P.  Protein Sci.,  8, 1725 - 1732.	bind
32012	1	7842	5	13	NULL	NULL	NULL	VEGF	GP		bind					KDR	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_8_832_s_255	9776730	33  Functional studies indicate that neuropilin enhanced the binding of VEGF to KDR resulting in VEGF-mediated chemotaxis.	bind
32013	2	7842	5	13	NULL	NULL	NULL	neuropilin	GP		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_8_832_s_255	9776730	33  Functional studies indicate that neuropilin enhanced the binding of VEGF to KDR resulting in VEGF-mediated chemotaxis.	bind
32014	4	7842	5	13	NULL	NULL	NULL	statement 2	Process		results in					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_8_832_s_255	9776730	33  Functional studies indicate that neuropilin enhanced the binding of VEGF to KDR resulting in VEGF-mediated chemotaxis.	bind
47359	3	7842	5	13	NULL	NULL	NULL	VEGF	GP		mediates					chemotaxis	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_8_832_s_255	9776730	33  Functional studies indicate that neuropilin enhanced the binding of VEGF to KDR resulting in VEGF-mediated chemotaxis.	bind
24788	1	7842	6	NULL	NULL	0	NULL	VEGF	NULL		bind	NULL				KDR	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_8_832_s_255	9776730	33  Functional studies indicate that neuropilin enhanced the binding of VEGF to KDR resulting in VEGF-mediated chemotaxis.	bind
24789	2	7842	6	NULL	NULL	0	NULL	neuropilin	NULL		enhance	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_8_832_s_255	9776730	33  Functional studies indicate that neuropilin enhanced the binding of VEGF to KDR resulting in VEGF-mediated chemotaxis.	bind
24790	4	7842	6	10	NULL	0	NULL	statement 2	NULL		results in	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_8_832_s_255	9776730	33  Functional studies indicate that neuropilin enhanced the binding of VEGF to KDR resulting in VEGF-mediated chemotaxis.	bind
47360	3	7842	6	10	NULL	0	NULL	VEGF	NULL		mediates	NULL				chemotaxis	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_8_832_s_255	9776730	33  Functional studies indicate that neuropilin enhanced the binding of VEGF to KDR resulting in VEGF-mediated chemotaxis.	bind
32015	1	7843	5	13	NULL	NULL	NULL	c-Myc	GP	induction of	leads to					RB	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_7_820_s_47	10205150	33  Induction of c-Myc can lead to rapid phosphorylation of RB and activation of both cyclin D1- and cyclin E-associated kinases in the absence of significant changes in the absolute amounts of cyclin-cdk complexes.	bind
32016	2	7843	5	13	NULL	NULL	NULL	c-Myc	GP	induction of	activates					cyclin E-associated kinases	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_7_820_s_47	10205150	33  Induction of c-Myc can lead to rapid phosphorylation of RB and activation of both cyclin D1- and cyclin E-associated kinases in the absence of significant changes in the absolute amounts of cyclin-cdk complexes.	bind
32017	3	7843	5	13	NULL	NULL	NULL	c-Myc	GP	induction of	activates					cyclin D1-associated kinases	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_7_820_s_47	10205150	33  Induction of c-Myc can lead to rapid phosphorylation of RB and activation of both cyclin D1- and cyclin E-associated kinases in the absence of significant changes in the absolute amounts of cyclin-cdk complexes.	bind
32018	4	7843	5	13	NULL	NULL	NULL	statement 1	Process		absence of					cyclin-cdk complexes	GP	significant changes in			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_7_820_s_47	10205150	33  Induction of c-Myc can lead to rapid phosphorylation of RB and activation of both cyclin D1- and cyclin E-associated kinases in the absence of significant changes in the absolute amounts of cyclin-cdk complexes.	bind
32019	5	7843	5	13	NULL	NULL	NULL	statement 2	Process		absence of					cyclin-cdk complexes	GP	significant changes in			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_7_820_s_47	10205150	33  Induction of c-Myc can lead to rapid phosphorylation of RB and activation of both cyclin D1- and cyclin E-associated kinases in the absence of significant changes in the absolute amounts of cyclin-cdk complexes.	bind
32020	6	7843	5	13	NULL	NULL	NULL	statement 3	Process		absence of					cyclin-cdk complexes	GP	significant changes in			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_7_820_s_47	10205150	33  Induction of c-Myc can lead to rapid phosphorylation of RB and activation of both cyclin D1- and cyclin E-associated kinases in the absence of significant changes in the absolute amounts of cyclin-cdk complexes.	bind
24792	1	7843	6	NULL	NULL	0	NULL	c-Myc	NULL	induction of	lead to	NULL				RB	NULL	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_circulationres_84_7_820_s_47	10205150	33  Induction of c-Myc can lead to rapid phosphorylation of RB and activation of both cyclin D1- and cyclin E-associated kinases in the absence of significant changes in the absolute amounts of cyclin-cdk complexes.	bind
24793	2	7843	6	NULL	NULL	0	NULL	c-Myc	NULL	induction of	results in	NULL				cyclin D1 associated kinases	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_circulationres_84_7_820_s_47	10205150	33  Induction of c-Myc can lead to rapid phosphorylation of RB and activation of both cyclin D1- and cyclin E-associated kinases in the absence of significant changes in the absolute amounts of cyclin-cdk complexes.	bind
24794	3	7843	6	NULL	NULL	0	NULL	c-Myc	NULL	induction of	results in	NULL				cyclin E-associated kinases	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_circulationres_84_7_820_s_47	10205150	33  Induction of c-Myc can lead to rapid phosphorylation of RB and activation of both cyclin D1- and cyclin E-associated kinases in the absence of significant changes in the absolute amounts of cyclin-cdk complexes.	bind
38773	4	7843	6	10	NULL	0	NULL	statement 1	NULL		occurs in absence of	NULL				cyclin-cdk complexes	NULL	significant changes in 			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_7_820_s_47	10205150	33  Induction of c-Myc can lead to rapid phosphorylation of RB and activation of both cyclin D1- and cyclin E-associated kinases in the absence of significant changes in the absolute amounts of cyclin-cdk complexes.	bind
38775	5	7843	6	10	NULL	0	NULL	statement 2	NULL		occurs in absence of	NULL				cyclin-cdk complexes	NULL	significant changes in 			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_7_820_s_47	10205150	33  Induction of c-Myc can lead to rapid phosphorylation of RB and activation of both cyclin D1- and cyclin E-associated kinases in the absence of significant changes in the absolute amounts of cyclin-cdk complexes.	bind
38776	6	7843	6	10	NULL	0	NULL	statement 3	NULL		occurs in absence of	NULL				cyclin-cdk complexes	NULL	significant changes in 			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_7_820_s_47	10205150	33  Induction of c-Myc can lead to rapid phosphorylation of RB and activation of both cyclin D1- and cyclin E-associated kinases in the absence of significant changes in the absolute amounts of cyclin-cdk complexes.	bind
32021	1	7844	5	13	NULL	NULL	NULL	PH1-IgG1 antibody	GP		bind		specifically			tumor	MedicalFinding				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1597_s_246	12000712	33  Summarized, the staining pattern of the PH1 epitope is only moderately different from staining patterns of other glycosylation-sensitive antibodies, it thus can be expected that the PH1-IgG1 antibody will specifically bind to tumor  in vivo.	bind
24795	1	7844	6	NULL	NULL	0	NULL	PH1-IgG1 antibody	NULL		bind	NULL	specifically			tumor	NULL				NULL	in vivo	0	NULL	NULL	NULL	gw60_amjpathol_160_5_1597_s_246	12000712	33  Summarized, the staining pattern of the PH1 epitope is only moderately different from staining patterns of other glycosylation-sensitive antibodies, it thus can be expected that the PH1-IgG1 antibody will specifically bind to tumor  in vivo.	bind
33804	1	7846	5	13	NULL	NULL	NULL	matrix proteins	GP		are scaffold for					tissue formation	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_1_217_s_216	12107106	33  These matrix proteins are the scaffold for tissue formation and growth, initiate intercellular signaling events through binding to cell receptor (integrins), and bind to growth factors and thus supply sustained concentration of these factors for epithelial cell migration, proliferation, and differentiation.	bind
33805	2	7846	5	13	NULL	NULL	NULL	matrix proteins	GP		are scaffold for					growth	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_1_217_s_216	12107106	33  These matrix proteins are the scaffold for tissue formation and growth, initiate intercellular signaling events through binding to cell receptor (integrins), and bind to growth factors and thus supply sustained concentration of these factors for epithelial cell migration, proliferation, and differentiation.	bind
33806	3	7846	5	13	NULL	NULL	NULL	matrix proteins	GP		bind					integrins	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_1_217_s_216	12107106	33  These matrix proteins are the scaffold for tissue formation and growth, initiate intercellular signaling events through binding to cell receptor (integrins), and bind to growth factors and thus supply sustained concentration of these factors for epithelial cell migration, proliferation, and differentiation.	bind
33807	4	7846	5	13	NULL	NULL	NULL	matrix proteins	GP		initiates					signaling events	Process	intercellular			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_1_217_s_216	12107106	33  These matrix proteins are the scaffold for tissue formation and growth, initiate intercellular signaling events through binding to cell receptor (integrins), and bind to growth factors and thus supply sustained concentration of these factors for epithelial cell migration, proliferation, and differentiation.	bind
33808	5	7846	5	13	NULL	NULL	NULL	statement 4	Process		occurs through					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_1_217_s_216	12107106	33  These matrix proteins are the scaffold for tissue formation and growth, initiate intercellular signaling events through binding to cell receptor (integrins), and bind to growth factors and thus supply sustained concentration of these factors for epithelial cell migration, proliferation, and differentiation.	bind
33809	6	7846	5	13	NULL	NULL	NULL	matrix proteins	GP		bind					growth factors	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_1_217_s_216	12107106	33  These matrix proteins are the scaffold for tissue formation and growth, initiate intercellular signaling events through binding to cell receptor (integrins), and bind to growth factors and thus supply sustained concentration of these factors for epithelial cell migration, proliferation, and differentiation.	bind
33810	7	7846	5	13	NULL	NULL	NULL	statement 6	Process		plays a role in					epithelial cell	Cell	migration of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_1_217_s_216	12107106	33  These matrix proteins are the scaffold for tissue formation and growth, initiate intercellular signaling events through binding to cell receptor (integrins), and bind to growth factors and thus supply sustained concentration of these factors for epithelial cell migration, proliferation, and differentiation.	bind
33811	8	7846	5	13	NULL	NULL	NULL	statement 6	Process		plays a role in					epithelial cell	Chemical	proliferation of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_1_217_s_216	12107106	33  These matrix proteins are the scaffold for tissue formation and growth, initiate intercellular signaling events through binding to cell receptor (integrins), and bind to growth factors and thus supply sustained concentration of these factors for epithelial cell migration, proliferation, and differentiation.	bind
33812	9	7846	5	13	NULL	NULL	NULL	statement 6	Process		plays a role in					epithelial cell	Cell	differentiation of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_1_217_s_216	12107106	33  These matrix proteins are the scaffold for tissue formation and growth, initiate intercellular signaling events through binding to cell receptor (integrins), and bind to growth factors and thus supply sustained concentration of these factors for epithelial cell migration, proliferation, and differentiation.	bind
24925	1	7846	6	NULL	NULL	0	NULL	matrix proteins	NULL		are scaffold for	NULL				tissue formation	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_1_217_s_216	12107106	33  These matrix proteins are the scaffold for tissue formation and growth, initiate intercellular signaling events through binding to cell receptor (integrins), and bind to growth factors and thus supply sustained concentration of these factors for epithelial cell migration, proliferation, and differentiation.	bind
24926	2	7846	6	NULL	NULL	0	NULL	matrix proteins	NULL		are scaffold for	NULL				tissue growth	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_1_217_s_216	12107106	33  These matrix proteins are the scaffold for tissue formation and growth, initiate intercellular signaling events through binding to cell receptor (integrins), and bind to growth factors and thus supply sustained concentration of these factors for epithelial cell migration, proliferation, and differentiation.	bind
24927	3	7846	6	NULL	NULL	0	NULL	matrix proteins	NULL		bind	NULL				cell receptor (integrins)	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_1_217_s_216	12107106	33  These matrix proteins are the scaffold for tissue formation and growth, initiate intercellular signaling events through binding to cell receptor (integrins), and bind to growth factors and thus supply sustained concentration of these factors for epithelial cell migration, proliferation, and differentiation.	bind
24928	4	7846	6	NULL	NULL	0	NULL	matrix proteins	NULL		bind	NULL				growth factors	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_1_217_s_216	12107106	33  These matrix proteins are the scaffold for tissue formation and growth, initiate intercellular signaling events through binding to cell receptor (integrins), and bind to growth factors and thus supply sustained concentration of these factors for epithelial cell migration, proliferation, and differentiation.	bind
32201	1	7847	5	13	NULL	NULL	NULL	LDL ligand	GP		bind					CRP	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2372_s_190	15486314	33 (2) Does ligand (for example, LDL) binding to CRP increase its affinity to Fc receptors?	bind
24796	1	7847	6	10	NULL	0	NULL	LDL ligand			bind					CRP					NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_12_2372_s_190	15486314	33 (2) Does ligand (for example, LDL) binding to CRP increase its affinity to Fc receptors?	bind
32202	1	7848	5	13	NULL	NULL	NULL	Hh	GP		bind					Ptc1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_113_20_2413_s_338	16702471	33 After Hh binds Ptc1, subsequent activation of Smo initiates signaling events that lead to the regulation of transcriptional factors belonging to the Gli family, which modify the expression of downstream target genes of the Hh pathway, including  Ptch and  Gli themselves.	bind
32203	2	7848	5	13	NULL	NULL	NULL	statement 1	Process		activates		subsequently			Smo	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_113_20_2413_s_338	16702471	33 After Hh binds Ptc1, subsequent activation of Smo initiates signaling events that lead to the regulation of transcriptional factors belonging to the Gli family, which modify the expression of downstream target genes of the Hh pathway, including  Ptch and  Gli themselves.	bind
32204	3	7848	5	13	NULL	NULL	NULL	statement 2	Process		initiates					signaling events	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_113_20_2413_s_338	16702471	33 After Hh binds Ptc1, subsequent activation of Smo initiates signaling events that lead to the regulation of transcriptional factors belonging to the Gli family, which modify the expression of downstream target genes of the Hh pathway, including  Ptch and  Gli themselves.	bind
32205	4	7848	5	13	NULL	NULL	NULL	statement 3	Process		leads to					Gli family transcriptional factors 	GP	regulation of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_113_20_2413_s_338	16702471	33 After Hh binds Ptc1, subsequent activation of Smo initiates signaling events that lead to the regulation of transcriptional factors belonging to the Gli family, which modify the expression of downstream target genes of the Hh pathway, including  Ptch and  Gli themselves.	bind
32206	5	7848	5	13	NULL	NULL	NULL	Gli family transcriptional factors 	GP		modify					Ptch	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_113_20_2413_s_338	16702471	33 After Hh binds Ptc1, subsequent activation of Smo initiates signaling events that lead to the regulation of transcriptional factors belonging to the Gli family, which modify the expression of downstream target genes of the Hh pathway, including  Ptch and  Gli themselves.	bind
32207	6	7848	5	13	NULL	NULL	NULL	Gli family transcriptional factors  	GP		modify					Gli	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_113_20_2413_s_338	16702471	33 After Hh binds Ptc1, subsequent activation of Smo initiates signaling events that lead to the regulation of transcriptional factors belonging to the Gli family, which modify the expression of downstream target genes of the Hh pathway, including  Ptch and  Gli themselves.	bind
32208	7	7848	5	13	NULL	NULL	NULL	Ptch	GP		is a type of					downstream target genes of Hh pathway	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_113_20_2413_s_338	16702471	33 After Hh binds Ptc1, subsequent activation of Smo initiates signaling events that lead to the regulation of transcriptional factors belonging to the Gli family, which modify the expression of downstream target genes of the Hh pathway, including  Ptch and  Gli themselves.	bind
32209	8	7848	5	13	NULL	NULL	NULL	Gli	GP		is a type of					downstream target genes of Hh pathway	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_113_20_2413_s_338	16702471	33 After Hh binds Ptc1, subsequent activation of Smo initiates signaling events that lead to the regulation of transcriptional factors belonging to the Gli family, which modify the expression of downstream target genes of the Hh pathway, including  Ptch and  Gli themselves.	bind
24881	1	7848	6	NULL	NULL	0	NULL	Hh	NULL		bind	NULL				Ptc1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_113_20_2413_s_338	16702471	33 After Hh binds Ptc1, subsequent activation of Smo initiates signaling events that lead to the regulation of transcriptional factors belonging to the Gli family, which modify the expression of downstream target genes of the Hh pathway, including  Ptch and  Gli themselves.	bind
24882	3	7848	6	10	NULL	0	NULL	statement 2	NULL		initiates	NULL				signaling events	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulation_113_20_2413_s_338	16702471	33 After Hh binds Ptc1, subsequent activation of Smo initiates signaling events that lead to the regulation of transcriptional factors belonging to the Gli family, which modify the expression of downstream target genes of the Hh pathway, including  Ptch and  Gli themselves.	bind
24883	2	7848	6	10	NULL	0	NULL	statement 1	NULL		activates	NULL	subsequently			Smo	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulation_113_20_2413_s_338	16702471	33 After Hh binds Ptc1, subsequent activation of Smo initiates signaling events that lead to the regulation of transcriptional factors belonging to the Gli family, which modify the expression of downstream target genes of the Hh pathway, including  Ptch and  Gli themselves.	bind
24884	5	7848	6	10	NULL	0	NULL	statement 4	NULL		modify the	NULL				Ptch	NULL	expression of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_113_20_2413_s_338	16702471	33 After Hh binds Ptc1, subsequent activation of Smo initiates signaling events that lead to the regulation of transcriptional factors belonging to the Gli family, which modify the expression of downstream target genes of the Hh pathway, including  Ptch and  Gli themselves.	bind
24885	6	7848	6	10	NULL	0	NULL	statement 4	NULL		modify the 	NULL				Gli	NULL	expression of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_113_20_2413_s_338	16702471	33 After Hh binds Ptc1, subsequent activation of Smo initiates signaling events that lead to the regulation of transcriptional factors belonging to the Gli family, which modify the expression of downstream target genes of the Hh pathway, including  Ptch and  Gli themselves.	bind
24886	7	7848	6	10	NULL	0	NULL	Ptch	NULL		is a type of	NULL				target gene of Hh pathway	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulation_113_20_2413_s_338	16702471	33 After Hh binds Ptc1, subsequent activation of Smo initiates signaling events that lead to the regulation of transcriptional factors belonging to the Gli family, which modify the expression of downstream target genes of the Hh pathway, including  Ptch and  Gli themselves.	bind
24887	8	7848	6	10	NULL	0	NULL	Gli	NULL		is a type of	NULL				target gene of Hh pathway	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulation_113_20_2413_s_338	16702471	33 After Hh binds Ptc1, subsequent activation of Smo initiates signaling events that lead to the regulation of transcriptional factors belonging to the Gli family, which modify the expression of downstream target genes of the Hh pathway, including  Ptch and  Gli themselves.	bind
47361	4	7848	6	10	NULL	0	NULL	statement 3	NULL		lead to	NULL				Gli family transcriptional factors 	NULL	regulation of			NULL		0	NULL	NULL	NULL	gw70_circulation_113_20_2413_s_338	16702471	33 After Hh binds Ptc1, subsequent activation of Smo initiates signaling events that lead to the regulation of transcriptional factors belonging to the Gli family, which modify the expression of downstream target genes of the Hh pathway, including  Ptch and  Gli themselves.	bind
32210	1	7849	5	13	NULL	NULL	NULL	CBP	GP		bind					AR	GP		LBD		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_48_31853_s_175	9822653	33 and  34), we have found that CBP can bind to both the NTD and LBD of AR.	bind
38968	2	7849	5	13	NULL	NULL	NULL	CBP	GP		bind					AR	GP		LBD		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_48_31853_s_175	9822653	33 and  34), we have found that CBP can bind to both the NTD and LBD of AR.	bind
24929	1	7849	6	NULL	NULL	0	NULL	CBP	NULL		bind	NULL				AR	NULL		NTD		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_48_31853_s_175	9822653	33 and  34), we have found that CBP can bind to both the NTD and LBD of AR.	bind
24930	2	7849	6	NULL	NULL	0	NULL	CBP	NULL		bind	NULL				AR	NULL		LBD		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_48_31853_s_175	9822653	33 and  34), we have found that CBP can bind to both the NTD and LBD of AR.	bind
32211	1	7850	5	13	NULL	NULL	NULL	adenosine	NucleicAcid		bind					A2A receptors	GP				NULL	neutrophils	NULL	NULL	NULL	NULL	gw70_circulationres_95_8_814_s_180	15358667	33 In neutrophils, adenosine binding to A2A receptors has been shown to counteract the stimulation of VLA-4 expression and binding to VCAM-1 by chemoattractants via a cAMP-mediated pathway.	bind
32212	2	7850	5	13	NULL	NULL	NULL	statement 1	Process		counteract					VLA-4 	GP	stimulation of;;expression of			NULL	neutrophils	NULL	NULL	NULL	NULL	gw70_circulationres_95_8_814_s_180	15358667	33 In neutrophils, adenosine binding to A2A receptors has been shown to counteract the stimulation of VLA-4 expression and binding to VCAM-1 by chemoattractants via a cAMP-mediated pathway.	bind
32213	3	7850	5	13	NULL	NULL	NULL	chemoattractants	GP		bind					VCAM-1	GP				NULL	neutrophils	NULL	NULL	NULL	NULL	gw70_circulationres_95_8_814_s_180	15358667	33 In neutrophils, adenosine binding to A2A receptors has been shown to counteract the stimulation of VLA-4 expression and binding to VCAM-1 by chemoattractants via a cAMP-mediated pathway.	bind
32214	4	7850	5	13	NULL	NULL	NULL	statement 3	Process		is mediated by					cAMP-pathway	Process				NULL	neutrophils	NULL	NULL	NULL	NULL	gw70_circulationres_95_8_814_s_180	15358667	33 In neutrophils, adenosine binding to A2A receptors has been shown to counteract the stimulation of VLA-4 expression and binding to VCAM-1 by chemoattractants via a cAMP-mediated pathway.	bind
24931	1	7850	6	NULL	NULL	0	NULL	adenosine	NULL		bind	NULL				A2A receptors	NULL				NULL	neutrophils	0	NULL	NULL	NULL	gw70_circulationres_95_8_814_s_180	15358667	33 In neutrophils, adenosine binding to A2A receptors has been shown to counteract the stimulation of VLA-4 expression and binding to VCAM-1 by chemoattractants via a cAMP-mediated pathway.	bind
24932	2	7850	6	10	NULL	0	NULL	chemoattractants	NULL		bind	NULL				VCAM-1	NULL				NULL	neutrophils	NULL	NULL	NULL	NULL	gw70_circulationres_95_8_814_s_180	15358667	33 In neutrophils, adenosine binding to A2A receptors has been shown to counteract the stimulation of VLA-4 expression and binding to VCAM-1 by chemoattractants via a cAMP-mediated pathway.	bind
24933	3	7850	6	10	NULL	0	NULL	statement 1	NULL		counteracts	NULL				VLA-4	NULL	stimulation of;; expression of			NULL	neutrophils	NULL	NULL	NULL	NULL	gw70_circulationres_95_8_814_s_180	15358667	33 In neutrophils, adenosine binding to A2A receptors has been shown to counteract the stimulation of VLA-4 expression and binding to VCAM-1 by chemoattractants via a cAMP-mediated pathway.	bind
24934	4	7850	6	NULL	NULL	0	NULL	statement 2	NULL		is mediated by	NULL				cAMP pathway	NULL				NULL	neutrophils	NULL	NULL	NULL	NULL	gw70_circulationres_95_8_814_s_180	15358667	33 In neutrophils, adenosine binding to A2A receptors has been shown to counteract the stimulation of VLA-4 expression and binding to VCAM-1 by chemoattractants via a cAMP-mediated pathway.	bind
32215	1	7851	5	13	NULL	NULL	NULL	LDLR	GP		bind				promoter	SREBP-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_164	15178557	33 It has been suggested that in LDLR promoter, the respective directional binding of SREBP-2 and Sp1 to their sites, which are head to head in repeats 2 and 3, allows the interaction of SREBP-2 with the N-terminal region of Sp1 and facilitates Sp1 recruitment 28 ( Figure 5).	bind
32216	2	7851	5	13	NULL	NULL	NULL	LDLR	GP		bind				promoter	Sp1	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_164	15178557	33 It has been suggested that in LDLR promoter, the respective directional binding of SREBP-2 and Sp1 to their sites, which are head to head in repeats 2 and 3, allows the interaction of SREBP-2 with the N-terminal region of Sp1 and facilitates Sp1 recruitment 28 ( Figure 5).	bind
32217	3	7851	5	13	NULL	NULL	NULL	SREBP-2	GP		interacts with					Sp1	GP		N-terminal region		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_164	15178557	33 It has been suggested that in LDLR promoter, the respective directional binding of SREBP-2 and Sp1 to their sites, which are head to head in repeats 2 and 3, allows the interaction of SREBP-2 with the N-terminal region of Sp1 and facilitates Sp1 recruitment 28 ( Figure 5).	bind
32218	4	7851	5	13	NULL	NULL	NULL	statement 1	Process		allows					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_164	15178557	33 It has been suggested that in LDLR promoter, the respective directional binding of SREBP-2 and Sp1 to their sites, which are head to head in repeats 2 and 3, allows the interaction of SREBP-2 with the N-terminal region of Sp1 and facilitates Sp1 recruitment 28 ( Figure 5).	bind
32219	5	7851	5	13	NULL	NULL	NULL	statement 2	Process		allows					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_164	15178557	33 It has been suggested that in LDLR promoter, the respective directional binding of SREBP-2 and Sp1 to their sites, which are head to head in repeats 2 and 3, allows the interaction of SREBP-2 with the N-terminal region of Sp1 and facilitates Sp1 recruitment 28 ( Figure 5).	bind
32220	6	7851	5	13	NULL	NULL	NULL	statement 1	Process		facilitate					Sp1	GP	recruitment of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_164	15178557	33 It has been suggested that in LDLR promoter, the respective directional binding of SREBP-2 and Sp1 to their sites, which are head to head in repeats 2 and 3, allows the interaction of SREBP-2 with the N-terminal region of Sp1 and facilitates Sp1 recruitment 28 ( Figure 5).	bind
32221	7	7851	5	13	NULL	NULL	NULL	statement 2	Process		facilitate					Sp1	GP	recruitment of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_164	15178557	33 It has been suggested that in LDLR promoter, the respective directional binding of SREBP-2 and Sp1 to their sites, which are head to head in repeats 2 and 3, allows the interaction of SREBP-2 with the N-terminal region of Sp1 and facilitates Sp1 recruitment 28 ( Figure 5).	bind
24936	1	7851	6	NULL	NULL	0	NULL	SREBP-2	NULL		bind	NULL				Sp1	NULL		N-terminal region		NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_164	15178557	33 It has been suggested that in LDLR promoter, the respective directional binding of SREBP-2 and Sp1 to their sites, which are head to head in repeats 2 and 3, allows the interaction of SREBP-2 with the N-terminal region of Sp1 and facilitates Sp1 recruitment 28 ( Figure 5).	bind
24937	2	7851	6	NULL	NULL	0	NULL	SREBP-2	NULL		bind	NULL				LDLR	NULL			site of promoter	NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_164	15178557	33 It has been suggested that in LDLR promoter, the respective directional binding of SREBP-2 and Sp1 to their sites, which are head to head in repeats 2 and 3, allows the interaction of SREBP-2 with the N-terminal region of Sp1 and facilitates Sp1 recruitment 28 ( Figure 5).	bind
24938	3	7851	6	NULL	NULL	0	NULL	Sp1	NULL		bind	NULL				LDLR	NULL			site of promoter	NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_164	15178557	33 It has been suggested that in LDLR promoter, the respective directional binding of SREBP-2 and Sp1 to their sites, which are head to head in repeats 2 and 3, allows the interaction of SREBP-2 with the N-terminal region of Sp1 and facilitates Sp1 recruitment 28 ( Figure 5).	bind
24941	4	7851	6	NULL	NULL	0	NULL	LDLR	NULL		is located on	NULL			SREBP-2 binding site		NULL			repeat 2	NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_164	15178557	33 It has been suggested that in LDLR promoter, the respective directional binding of SREBP-2 and Sp1 to their sites, which are head to head in repeats 2 and 3, allows the interaction of SREBP-2 with the N-terminal region of Sp1 and facilitates Sp1 recruitment 28 ( Figure 5).	bind
24942	5	7851	6	NULL	NULL	0	NULL	LDLR	NULL		is located on	NULL			Sp1 binding site		NULL			repeat 3	NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_164	15178557	33 It has been suggested that in LDLR promoter, the respective directional binding of SREBP-2 and Sp1 to their sites, which are head to head in repeats 2 and 3, allows the interaction of SREBP-2 with the N-terminal region of Sp1 and facilitates Sp1 recruitment 28 ( Figure 5).	bind
24943	6	7851	6	NULL	NULL	0	NULL	statement 2	NULL		allows	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_164	15178557	33 It has been suggested that in LDLR promoter, the respective directional binding of SREBP-2 and Sp1 to their sites, which are head to head in repeats 2 and 3, allows the interaction of SREBP-2 with the N-terminal region of Sp1 and facilitates Sp1 recruitment 28 ( Figure 5).	bind
24944	7	7851	6	NULL	NULL	0	NULL	statement 3	NULL		allows	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_164	15178557	33 It has been suggested that in LDLR promoter, the respective directional binding of SREBP-2 and Sp1 to their sites, which are head to head in repeats 2 and 3, allows the interaction of SREBP-2 with the N-terminal region of Sp1 and facilitates Sp1 recruitment 28 ( Figure 5).	bind
24945	8	7851	6	NULL	NULL	0	NULL	statement 2	NULL		facilitate	NULL				Sp1	NULL	recruitment of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_164	15178557	33 It has been suggested that in LDLR promoter, the respective directional binding of SREBP-2 and Sp1 to their sites, which are head to head in repeats 2 and 3, allows the interaction of SREBP-2 with the N-terminal region of Sp1 and facilitates Sp1 recruitment 28 ( Figure 5).	bind
24946	9	7851	6	NULL	NULL	0	NULL	statement 3	NULL		facilitate	NULL				Sp1	NULL	recruitment of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1454_s_164	15178557	33 It has been suggested that in LDLR promoter, the respective directional binding of SREBP-2 and Sp1 to their sites, which are head to head in repeats 2 and 3, allows the interaction of SREBP-2 with the N-terminal region of Sp1 and facilitates Sp1 recruitment 28 ( Figure 5).	bind
32222	1	7852	5	13	NULL	NULL	NULL	L-4F	GP		bind					LPS	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_3_236_s_240	16002747	33 Our data suggest that L-4F binds LPS and alters its aggregation state.	bind
32223	2	7852	5	13	NULL	NULL	NULL	statement 1	Process		alters					LPS	Chemical	aggregation state of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_3_236_s_240	16002747	33 Our data suggest that L-4F binds LPS and alters its aggregation state.	bind
24939	1	7852	6	NULL	NULL	0	NULL	L-4F	NULL		bind	NULL				LPS	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_3_236_s_240	16002747	33 Our data suggest that L-4F binds LPS and alters its aggregation state.	bind
24940	2	7852	6	NULL	NULL	0	NULL	statement 1	NULL		alters	NULL				LPS	NULL	aggregation state of 			NULL		0	NULL	NULL	NULL	gw70_circulationres_97_3_236_s_240	16002747	33 Our data suggest that L-4F binds LPS and alters its aggregation state.	bind
32224	1	7853	5	13	NULL	NULL	NULL	NRRE-1	GP		is a type of					complex response element	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_6_568_s_84	15375023	33 The complex response element (NRRE-1) conferring PPARalpha responsiveness binds several NRs and dictates the developmental and FA responsiveness of the MCAD gene.	bind
32225	2	7853	5	13	NULL	NULL	NULL				confers				NRRE-1	PPARalpha	GP	responsiveness of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_6_568_s_84	15375023	33 The complex response element (NRRE-1) conferring PPARalpha responsiveness binds several NRs and dictates the developmental and FA responsiveness of the MCAD gene.	bind
32226	3	7853	5	13	NULL	NULL	NULL				bind				NRRE-1	NRs	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_6_568_s_84	15375023	33 The complex response element (NRRE-1) conferring PPARalpha responsiveness binds several NRs and dictates the developmental and FA responsiveness of the MCAD gene.	bind
32227	4	7853	5	13	NULL	NULL	NULL	statement 3	Process		dictates					MCAD gene	GP	development of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_6_568_s_84	15375023	33 The complex response element (NRRE-1) conferring PPARalpha responsiveness binds several NRs and dictates the developmental and FA responsiveness of the MCAD gene.	bind
32228	5	7853	5	13	NULL	NULL	NULL	statement 3	Process		dictates					MCAD gene	GP	FA responsiveness of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_6_568_s_84	15375023	33 The complex response element (NRRE-1) conferring PPARalpha responsiveness binds several NRs and dictates the developmental and FA responsiveness of the MCAD gene.	bind
24958	1	7853	6	10	NULL	0	NULL	NRRE-1	NULL		is a type of	NULL				complex response element	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_6_568_s_84	15375023	33 The complex response element (NRRE-1) conferring PPARalpha responsiveness binds several NRs and dictates the developmental and FA responsiveness of the MCAD gene.	bind
24977	2	7853	6	NULL	NULL	0	NULL		NULL		confers	NULL			NRRE-1	PPARalpha	NULL	 responsiveness of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_6_568_s_84	15375023	33 The complex response element (NRRE-1) conferring PPARalpha responsiveness binds several NRs and dictates the developmental and FA responsiveness of the MCAD gene.	bind
24978	3	7853	6	NULL	NULL	0	NULL		NULL		bind	NULL			NRRE-1	NRs	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_6_568_s_84	15375023	33 The complex response element (NRRE-1) conferring PPARalpha responsiveness binds several NRs and dictates the developmental and FA responsiveness of the MCAD gene.	bind
24980	4	7853	6	NULL	NULL	0	NULL		NULL		dictates	NULL			NRRE-1	MCAD gene	NULL	developmental responsiveness of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_6_568_s_84	15375023	33 The complex response element (NRRE-1) conferring PPARalpha responsiveness binds several NRs and dictates the developmental and FA responsiveness of the MCAD gene.	bind
24981	5	7853	6	NULL	NULL	0	NULL		NULL		dictates	NULL			NRRE-1	MCAD gene	NULL	FA responsiveness of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_6_568_s_84	15375023	33 The complex response element (NRRE-1) conferring PPARalpha responsiveness binds several NRs and dictates the developmental and FA responsiveness of the MCAD gene.	bind
32229	1	7854	5	13	NULL	NULL	NULL	IGF-1	GP		bind					IGF-1 receptors	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_20_2588_s_172	15883206	33 We have previously shown that IGF-1 binding to the IGF-1 receptors results in a Ca2+-dependent positive inotropic effect.	bind
32230	2	7854	5	13	NULL	NULL	NULL	statement 1	Process		results in					inotropic effect	Process	positive			NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_20_2588_s_172	15883206	33 We have previously shown that IGF-1 binding to the IGF-1 receptors results in a Ca2+-dependent positive inotropic effect.	bind
32231	3	7854	5	13	NULL	NULL	NULL	statement 2	Process		is dependent on					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_20_2588_s_172	15883206	33 We have previously shown that IGF-1 binding to the IGF-1 receptors results in a Ca2+-dependent positive inotropic effect.	bind
24983	1	7854	6	NULL	NULL	0	NULL	IGF-1	NULL		bind	NULL				IGF-1 receptor	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_111_20_2588_s_172	15883206	33 We have previously shown that IGF-1 binding to the IGF-1 receptors results in a Ca2+-dependent positive inotropic effect.	bind
24984	2	7854	6	NULL	NULL	0	NULL	statement 1	NULL		results in	NULL				inotropic effect	NULL	positive			NULL		0	NULL	NULL	NULL	gw70_circulation_111_20_2588_s_172	15883206	33 We have previously shown that IGF-1 binding to the IGF-1 receptors results in a Ca2+-dependent positive inotropic effect.	bind
24985	3	7854	6	NULL	NULL	0	NULL	statement 2	NULL		is dependent on	NULL				Ca2+	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_111_20_2588_s_172	15883206	33 We have previously shown that IGF-1 binding to the IGF-1 receptors results in a Ca2+-dependent positive inotropic effect.	bind
32232	1	7855	5	13	NULL	NULL	NULL	Smad1	GP		does not bind									AGAC	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_10_992_s_110	16224060	33,34  However, Smad1 or Smad4 did not bind to the 3 AGAC and flanking &10 bp by EMSA (data not shown).	bind
32233	2	7855	5	13	NULL	NULL	NULL	Smad4	GP		does not bind									AGAC	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_10_992_s_110	16224060	33,34  However, Smad1 or Smad4 did not bind to the 3 AGAC and flanking &10 bp by EMSA (data not shown).	bind
24987	1	7855	6	10	NULL	0	NULL	Smad1	NULL		does not bind	NULL					NULL			AGAC	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_10_992_s_110	16224060	33,34  However, Smad1 or Smad4 did not bind to the 3 AGAC and flanking &10 bp by EMSA (data not shown).	bind
24988	2	7855	6	10	NULL	0	NULL	Smad4	NULL		does not bind	NULL					NULL			AGAC	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_10_992_s_110	16224060	33,34  However, Smad1 or Smad4 did not bind to the 3 AGAC and flanking &10 bp by EMSA (data not shown).	bind
32391	1	7856	5	13	NULL	NULL	NULL	nitric oxide	Chemical		inhibits					thrombus		formation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_454_s_168	15569820	33,34  Nitric oxide inhibits the formation of thrombus under high-shear flow 37 and attenuates agonist-induced upregulation of P-selectin and the binding of vWF to platelet GPIb complex by negatively regulating the cGMP in platelets.	bind
32392	2	7856	5	13	NULL	NULL	NULL	high-shear flow			is required for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_454_s_168	15569820	33,34  Nitric oxide inhibits the formation of thrombus under high-shear flow 37 and attenuates agonist-induced upregulation of P-selectin and the binding of vWF to platelet GPIb complex by negatively regulating the cGMP in platelets.	bind
32393	3	7856	5	13	NULL	NULL	NULL	agonist	Chemical		induces					P-selectin	GP	upregulation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_454_s_168	15569820	33,34  Nitric oxide inhibits the formation of thrombus under high-shear flow 37 and attenuates agonist-induced upregulation of P-selectin and the binding of vWF to platelet GPIb complex by negatively regulating the cGMP in platelets.	bind
32394	4	7856	5	13	NULL	NULL	NULL	nitric oxide	Chemical		attenuates					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_454_s_168	15569820	33,34  Nitric oxide inhibits the formation of thrombus under high-shear flow 37 and attenuates agonist-induced upregulation of P-selectin and the binding of vWF to platelet GPIb complex by negatively regulating the cGMP in platelets.	bind
32395	5	7856	5	13	NULL	NULL	NULL	VWF	GP		bind					platelet GPIb complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_454_s_168	15569820	33,34  Nitric oxide inhibits the formation of thrombus under high-shear flow 37 and attenuates agonist-induced upregulation of P-selectin and the binding of vWF to platelet GPIb complex by negatively regulating the cGMP in platelets.	bind
32396	6	7856	5	13	NULL	NULL	NULL	nitric oxide	Chemical		regulates		negatively			cGMP	Chemical				NULL	in platelets	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_454_s_168	15569820	33,34  Nitric oxide inhibits the formation of thrombus under high-shear flow 37 and attenuates agonist-induced upregulation of P-selectin and the binding of vWF to platelet GPIb complex by negatively regulating the cGMP in platelets.	bind
32397	7	7856	5	13	NULL	NULL	NULL	statement 6	Process		attenuates					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_454_s_168	15569820	33,34  Nitric oxide inhibits the formation of thrombus under high-shear flow 37 and attenuates agonist-induced upregulation of P-selectin and the binding of vWF to platelet GPIb complex by negatively regulating the cGMP in platelets.	bind
24989	1	7856	6	NULL	NULL	0	NULL	Nitric oxide	NULL		inhibits	NULL				thrombus	NULL	formation of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_454_s_168	15569820	33,34  Nitric oxide inhibits the formation of thrombus under high-shear flow 37 and attenuates agonist-induced upregulation of P-selectin and the binding of vWF to platelet GPIb complex by negatively regulating the cGMP in platelets.	bind
24990	2	7856	6	NULL	NULL	0	NULL	statement 1	NULL		occurs under	NULL				high shear flow	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_454_s_168	15569820	33,34  Nitric oxide inhibits the formation of thrombus under high-shear flow 37 and attenuates agonist-induced upregulation of P-selectin and the binding of vWF to platelet GPIb complex by negatively regulating the cGMP in platelets.	bind
24991	3	7856	6	NULL	NULL	0	NULL	vWF	NULL		bind	NULL				platelet GPIb complex	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_454_s_168	15569820	33,34  Nitric oxide inhibits the formation of thrombus under high-shear flow 37 and attenuates agonist-induced upregulation of P-selectin and the binding of vWF to platelet GPIb complex by negatively regulating the cGMP in platelets.	bind
24992	4	7856	6	NULL	NULL	0	NULL	agonist	NULL		induces	NULL				P-selectin	NULL	upregulation of 			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_454_s_168	15569820	33,34  Nitric oxide inhibits the formation of thrombus under high-shear flow 37 and attenuates agonist-induced upregulation of P-selectin and the binding of vWF to platelet GPIb complex by negatively regulating the cGMP in platelets.	bind
24994	5	7856	6	NULL	NULL	0	NULL	Nitric oxide	NULL		attenuates	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_454_s_168	15569820	33,34  Nitric oxide inhibits the formation of thrombus under high-shear flow 37 and attenuates agonist-induced upregulation of P-selectin and the binding of vWF to platelet GPIb complex by negatively regulating the cGMP in platelets.	bind
24997	6	7856	6	NULL	NULL	0	NULL	Nitric oxide	NULL		attenuates	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_454_s_168	15569820	33,34  Nitric oxide inhibits the formation of thrombus under high-shear flow 37 and attenuates agonist-induced upregulation of P-selectin and the binding of vWF to platelet GPIb complex by negatively regulating the cGMP in platelets.	bind
24999	7	7856	6	10	NULL	0	NULL	statement 6	NULL		regulates	NULL	negatively			cGMP 	NULL				NULL	in platelets	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_454_s_168	15569820	33,34  Nitric oxide inhibits the formation of thrombus under high-shear flow 37 and attenuates agonist-induced upregulation of P-selectin and the binding of vWF to platelet GPIb complex by negatively regulating the cGMP in platelets.	bind
32398	1	7857	5	13	NULL	NULL	NULL	decorin	GP		bind					PDGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_163_3_869_s_288	12937128	33,35  Decorin-PDGF binding and inhibition of PDGFR phosphorylation by decorin reported in this study indicate an additional mechanism of ECM regulation by decorin.	bind
32399	2	7857	5	13	NULL	NULL	NULL	decorin	GP		inhibits					PDGFR	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_163_3_869_s_288	12937128	33,35  Decorin-PDGF binding and inhibition of PDGFR phosphorylation by decorin reported in this study indicate an additional mechanism of ECM regulation by decorin.	bind
32400	3	7857	5	13	NULL	NULL	NULL	decorin	GP		regulates					ECM	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_163_3_869_s_288	12937128	33,35  Decorin-PDGF binding and inhibition of PDGFR phosphorylation by decorin reported in this study indicate an additional mechanism of ECM regulation by decorin.	bind
25000	1	7857	6	NULL	NULL	0	NULL	decorin	NULL		bind	NULL				PDGF	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_163_3_869_s_288	12937128	33,35  Decorin-PDGF binding and inhibition of PDGFR phosphorylation by decorin reported in this study indicate an additional mechanism of ECM regulation by decorin.	bind
25001	2	7857	6	NULL	NULL	0	NULL	decorin	NULL		inhibits	NULL				PDGFR	NULL	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_163_3_869_s_288	12937128	33,35  Decorin-PDGF binding and inhibition of PDGFR phosphorylation by decorin reported in this study indicate an additional mechanism of ECM regulation by decorin.	bind
25002	3	7857	6	NULL	NULL	0	NULL	decorin	NULL		regulates	NULL				ECM	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_163_3_869_s_288	12937128	33,35  Decorin-PDGF binding and inhibition of PDGFR phosphorylation by decorin reported in this study indicate an additional mechanism of ECM regulation by decorin.	bind
32401	1	7859	5	13	NULL	NULL	NULL	zinc finger/homeodomain protein	GP		bind									T3-response elements	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_24_4846_s_383	11121475	34       Cabanillas,A.M. and Darling,D.S. (1996) Alternative splicing gives rise to two isoforms of Zfhep, a zinc finger/homeodomain protein that binds  T3-response elements.	bind
38970	2	7859	5	13	NULL	NULL	NULL	Zfhep	GP		is a type of					zinc finger/homeodomain protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_24_4846_s_383	11121475	34       Cabanillas,A.M. and Darling,D.S. (1996) Alternative splicing gives rise to two isoforms of Zfhep, a zinc finger/homeodomain protein that binds  T3-response elements.	bind
25004	1	7859	6	13	NULL	NULL	NULL	Zfhep	GP		is a type of					zinc finger/homeodomain protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_24_4846_s_383	11121475	34       Cabanillas,A.M. and Darling,D.S. (1996) Alternative splicing gives rise to two isoforms of Zfhep, a zinc finger/homeodomain protein that binds  T3-response elements.	bind
25005	2	7859	6	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL					NULL			T3-response elements	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_24_4846_s_383	11121475	34       Cabanillas,A.M. and Darling,D.S. (1996) Alternative splicing gives rise to two isoforms of Zfhep, a zinc finger/homeodomain protein that binds  T3-response elements.	bind
25007	3	7859	6	NULL	NULL	0	NULL	Alternative splicing	NULL		gives rise to	NULL				Zfhep	NULL	two isoforms of 			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_24_4846_s_383	11121475	34       Cabanillas,A.M. and Darling,D.S. (1996) Alternative splicing gives rise to two isoforms of Zfhep, a zinc finger/homeodomain protein that binds  T3-response elements.	bind
32402	1	7860	5	13	NULL	NULL	NULL	Ni2+	Chemical		bind					polynucleotides	NucleicAcid	synthetic		regularly alternating purine - pyrimidine sequences	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2795_s_307	11433025	34       Kankia,B.I. (2000) Hydration effects of Ni2+ binding to synthetic polynucleotides with regularly alternating purine - pyrimidine sequences.	bind
25008	1	7860	6	NULL	NULL	0	NULL	Ni2+	NULL		bind	NULL				polynucleotides	NULL	synthetic		 regularly alternating purine - pyrimidine sequences	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2795_s_307	11433025	34       Kankia,B.I. (2000) Hydration effects of Ni2+ binding to synthetic polynucleotides with regularly alternating purine - pyrimidine sequences.	bind
32403	1	7861	5	13	NULL	NULL	NULL	U1A protein	GP	human	does not bind			C-terminal RNA binding domain		RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_550_s_360	11788718	34       Lu,J. and Hall,K.B. (1995) An RBD that does not bind RNA: NMR secondary structure determination and biochemical properties of the  C-terminal RNA binding domain from the human U1A protein.	bind
25010	1	7861	6	NULL	NULL	0	NULL	U1A protein	NULL	human	does not bind	NULL		C-terminal RNA binding domain		RNA	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_550_s_360	11788718	34       Lu,J. and Hall,K.B. (1995) An RBD that does not bind RNA: NMR secondary structure determination and biochemical properties of the  C-terminal RNA binding domain from the human U1A protein.	bind
32404	1	7862	5	13	NULL	NULL	NULL	SR protein	GP		bind		sequence-specific			RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_24_4822_s_354	11121472	34       Tacke,R., Chen,Y. and Manley,J.L. (1997) Sequence-specific RNA binding by an SR protein requires RS domain phosphorylation: creation of an SRp40-specific splicing enhancer.	bind
32405	2	7862	5	13	NULL	NULL	NULL			phosphorylation of	is required for			RS domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_24_4822_s_354	11121472	34       Tacke,R., Chen,Y. and Manley,J.L. (1997) Sequence-specific RNA binding by an SR protein requires RS domain phosphorylation: creation of an SRp40-specific splicing enhancer.	bind
25011	1	7862	6	NULL	NULL	0	NULL	SR protein	NULL		bind	NULL	sequence specifically			RNA	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_24_4822_s_354	11121472	34       Tacke,R., Chen,Y. and Manley,J.L. (1997) Sequence-specific RNA binding by an SR protein requires RS domain phosphorylation: creation of an SRp40-specific splicing enhancer.	bind
25012	2	7862	6	NULL	NULL	0	NULL	statement 1	NULL		requires	NULL					NULL	phosphorylation of	RS domain		NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_24_4822_s_354	11121472	34       Tacke,R., Chen,Y. and Manley,J.L. (1997) Sequence-specific RNA binding by an SR protein requires RS domain phosphorylation: creation of an SRp40-specific splicing enhancer.	bind
32406	1	7863	5	13	NULL	NULL	NULL	RNAI	GP		bind					RNAII	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_15_3145_s_368	11470871	34       Tomizawa,J. (1990) Control of ColE1 plasmid replication: intermediates in the binding of RNAI and RNAII.	bind
25013	1	7863	6	NULL	NULL	0	NULL	RNAI	NULL		bind	NULL				RNAII	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_15_3145_s_368	11470871	34       Tomizawa,J. (1990) Control of ColE1 plasmid replication: intermediates in the binding of RNAI and RNAII.	bind
32407	1	7864	5	13	NULL	NULL	NULL	heparin	Chemical		bind					platelet factor 4	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_9_2877_s_179	9386152	34  In addition, heparin binds to platelet factor 4, another alpha-granule constituent.	bind
32408	2	7864	5	13	NULL	NULL	NULL	platelet factor 4	GP		is a type of					alpha-granule constituent	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_9_2877_s_179	9386152	34  In addition, heparin binds to platelet factor 4, another alpha-granule constituent.	bind
25014	1	7864	6	NULL	NULL	0	NULL	heparin	NULL		bind	NULL				platelet factor 4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_96_9_2877_s_179	9386152	34  In addition, heparin binds to platelet factor 4, another alpha-granule constituent.	bind
25015	2	7864	6	10	NULL	0	NULL	platelet factor 4	NULL		is a type of	NULL				alpha-granule constituent	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_9_2877_s_179	9386152	34  In addition, heparin binds to platelet factor 4, another alpha-granule constituent.	bind
32409	1	7865	5	13	NULL	NULL	NULL	TNF-alpha	GP		bind					ECM	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_13	12000736	34  In addition, TNF-alpha bound to ECM exhibits biological activity, as demonstrated by findings that when bound to fibronectin, this cytokine modifies beta1-integrin-mediated adhesion of T lymphocytes, 31 provides a stop signal for migration of T cells, 32  and stimulates MMP-9 expression by monocytes.	bind
32410	2	7865	5	13	NULL	NULL	NULL	TNF-alpha	GP		bind					fibronectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_13	12000736	34  In addition, TNF-alpha bound to ECM exhibits biological activity, as demonstrated by findings that when bound to fibronectin, this cytokine modifies beta1-integrin-mediated adhesion of T lymphocytes, 31 provides a stop signal for migration of T cells, 32  and stimulates MMP-9 expression by monocytes.	bind
32411	3	7865	5	13	NULL	NULL	NULL	beta1-integrin	GP		mediates					T lymphocytes	Cell	adhesion of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_13	12000736	34  In addition, TNF-alpha bound to ECM exhibits biological activity, as demonstrated by findings that when bound to fibronectin, this cytokine modifies beta1-integrin-mediated adhesion of T lymphocytes, 31 provides a stop signal for migration of T cells, 32  and stimulates MMP-9 expression by monocytes.	bind
32412	4	7865	5	13	NULL	NULL	NULL	statement 2	Process		modify					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_13	12000736	34  In addition, TNF-alpha bound to ECM exhibits biological activity, as demonstrated by findings that when bound to fibronectin, this cytokine modifies beta1-integrin-mediated adhesion of T lymphocytes, 31 provides a stop signal for migration of T cells, 32  and stimulates MMP-9 expression by monocytes.	bind
32413	5	7865	5	13	NULL	NULL	NULL	statement 2	Process		stops					T cells	Cell	 signal for migration of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_13	12000736	34  In addition, TNF-alpha bound to ECM exhibits biological activity, as demonstrated by findings that when bound to fibronectin, this cytokine modifies beta1-integrin-mediated adhesion of T lymphocytes, 31 provides a stop signal for migration of T cells, 32  and stimulates MMP-9 expression by monocytes.	bind
32414	6	7865	5	13	NULL	NULL	NULL	monocytes	Cell		express					MMP-9	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_13	12000736	34  In addition, TNF-alpha bound to ECM exhibits biological activity, as demonstrated by findings that when bound to fibronectin, this cytokine modifies beta1-integrin-mediated adhesion of T lymphocytes, 31 provides a stop signal for migration of T cells, 32  and stimulates MMP-9 expression by monocytes.	bind
32415	7	7865	5	13	NULL	NULL	NULL	statement 2	Process		stimulates					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_13	12000736	34  In addition, TNF-alpha bound to ECM exhibits biological activity, as demonstrated by findings that when bound to fibronectin, this cytokine modifies beta1-integrin-mediated adhesion of T lymphocytes, 31 provides a stop signal for migration of T cells, 32  and stimulates MMP-9 expression by monocytes.	bind
25016	1	7865	6	NULL	NULL	0	NULL	TNF-alpha	NULL		bind	NULL				ECM	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_13	12000736	34  In addition, TNF-alpha bound to ECM exhibits biological activity, as demonstrated by findings that when bound to fibronectin, this cytokine modifies beta1-integrin-mediated adhesion of T lymphocytes, 31 provides a stop signal for migration of T cells, 32  and stimulates MMP-9 expression by monocytes.	bind
25017	2	7865	6	NULL	NULL	0	NULL	statement 1	NULL		exhibits	NULL				biological activity	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_13	12000736	34  In addition, TNF-alpha bound to ECM exhibits biological activity, as demonstrated by findings that when bound to fibronectin, this cytokine modifies beta1-integrin-mediated adhesion of T lymphocytes, 31 provides a stop signal for migration of T cells, 32  and stimulates MMP-9 expression by monocytes.	bind
25018	3	7865	6	NULL	NULL	0	NULL	TNF-alpha	NULL		bind	NULL				fibronectin	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_13	12000736	34  In addition, TNF-alpha bound to ECM exhibits biological activity, as demonstrated by findings that when bound to fibronectin, this cytokine modifies beta1-integrin-mediated adhesion of T lymphocytes, 31 provides a stop signal for migration of T cells, 32  and stimulates MMP-9 expression by monocytes.	bind
25019	4	7865	6	NULL	NULL	0	NULL	beta1 integrin	NULL		mediates	NULL				T lymphocytes	NULL	adhesion of 			NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_13	12000736	34  In addition, TNF-alpha bound to ECM exhibits biological activity, as demonstrated by findings that when bound to fibronectin, this cytokine modifies beta1-integrin-mediated adhesion of T lymphocytes, 31 provides a stop signal for migration of T cells, 32  and stimulates MMP-9 expression by monocytes.	bind
25020	5	7865	6	NULL	NULL	0	NULL	statement 3	NULL		modifies	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_13	12000736	34  In addition, TNF-alpha bound to ECM exhibits biological activity, as demonstrated by findings that when bound to fibronectin, this cytokine modifies beta1-integrin-mediated adhesion of T lymphocytes, 31 provides a stop signal for migration of T cells, 32  and stimulates MMP-9 expression by monocytes.	bind
25851	6	7865	6	NULL	NULL	0	NULL	statement 3	NULL		stops	NULL				T cells	NULL	migration of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_13	12000736	34  In addition, TNF-alpha bound to ECM exhibits biological activity, as demonstrated by findings that when bound to fibronectin, this cytokine modifies beta1-integrin-mediated adhesion of T lymphocytes, 31 provides a stop signal for migration of T cells, 32  and stimulates MMP-9 expression by monocytes.	bind
25852	7	7865	6	NULL	NULL	0	NULL	monocytes	NULL		express	NULL				MMP-9	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_13	12000736	34  In addition, TNF-alpha bound to ECM exhibits biological activity, as demonstrated by findings that when bound to fibronectin, this cytokine modifies beta1-integrin-mediated adhesion of T lymphocytes, 31 provides a stop signal for migration of T cells, 32  and stimulates MMP-9 expression by monocytes.	bind
25853	8	7865	6	NULL	NULL	0	NULL	TNF-alpha	NULL		stimulates	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_13	12000736	34  In addition, TNF-alpha bound to ECM exhibits biological activity, as demonstrated by findings that when bound to fibronectin, this cytokine modifies beta1-integrin-mediated adhesion of T lymphocytes, 31 provides a stop signal for migration of T cells, 32  and stimulates MMP-9 expression by monocytes.	bind
32416	1	7866	5	13	NULL	NULL	NULL	PlGF homodimers	GP		bind					VEGFR-1	GP				NULL	HUVEC	NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_993_s_349	11549592	34  Moreover, the fact that PlGF homodimers that bind to VEGFR-1 and PlGF:VEGF heterodimers that bind to VEGFR-2 induced tyrosine phosphorylation of a 38-kd protein in HUVECs whereas VEGF homodimers did not 29  supports the view that PlGF and VEGF can exert different biological actions through the same receptor.	bind
32418	2	7866	5	13	NULL	NULL	NULL	PlGF:VEGF heterodimers	GP		bind					VEGFR-2	GP				NULL	HUVEC	NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_993_s_349	11549592	34  Moreover, the fact that PlGF homodimers that bind to VEGFR-1 and PlGF:VEGF heterodimers that bind to VEGFR-2 induced tyrosine phosphorylation of a 38-kd protein in HUVECs whereas VEGF homodimers did not 29  supports the view that PlGF and VEGF can exert different biological actions through the same receptor.	bind
32419	3	7866	5	13	NULL	NULL	NULL	statement 1	Process		induces					38-kd protein	GP	phosphorylation of	tyrosine		NULL	in HUVECs 	NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_993_s_349	11549592	34  Moreover, the fact that PlGF homodimers that bind to VEGFR-1 and PlGF:VEGF heterodimers that bind to VEGFR-2 induced tyrosine phosphorylation of a 38-kd protein in HUVECs whereas VEGF homodimers did not 29  supports the view that PlGF and VEGF can exert different biological actions through the same receptor.	bind
32420	4	7866	5	13	NULL	NULL	NULL	statement 3	Process		induces					38-kd protein	GP	phosphorylation of	tyrosine		NULL	in HUVECs	NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_993_s_349	11549592	34  Moreover, the fact that PlGF homodimers that bind to VEGFR-1 and PlGF:VEGF heterodimers that bind to VEGFR-2 induced tyrosine phosphorylation of a 38-kd protein in HUVECs whereas VEGF homodimers did not 29  supports the view that PlGF and VEGF can exert different biological actions through the same receptor.	bind
25021	1	7866	6	10	NULL	0	NULL	PlGF homodimers			bind					VEGFR-1					NULL	HUVEC	NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_993_s_349	11549592	34  Moreover, the fact that PlGF homodimers that bind to VEGFR-1 and PlGF:VEGF heterodimers that bind to VEGFR-2 induced tyrosine phosphorylation of a 38-kd protein in HUVECs whereas VEGF homodimers did not 29  supports the view that PlGF and VEGF can exert different biological actions through the same receptor.	bind
25022	2	7866	6	10	NULL	0	NULL	PlGF:VEGF heterodimers			bind					VEGFR-2					NULL	HUVEC	NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_993_s_349	11549592	34  Moreover, the fact that PlGF homodimers that bind to VEGFR-1 and PlGF:VEGF heterodimers that bind to VEGFR-2 induced tyrosine phosphorylation of a 38-kd protein in HUVECs whereas VEGF homodimers did not 29  supports the view that PlGF and VEGF can exert different biological actions through the same receptor.	bind
25024	3	7866	6	NULL	NULL	0	NULL	statement 1	NULL		induces	NULL				38-kd protein	NULL	phosphorylation of	tyrosine		NULL	HUVEC	0	NULL	NULL	NULL	gw60_amjpathol_159_3_993_s_349	11549592	34  Moreover, the fact that PlGF homodimers that bind to VEGFR-1 and PlGF:VEGF heterodimers that bind to VEGFR-2 induced tyrosine phosphorylation of a 38-kd protein in HUVECs whereas VEGF homodimers did not 29  supports the view that PlGF and VEGF can exert different biological actions through the same receptor.	bind
25025	4	7866	6	NULL	NULL	0	NULL	statement 2	NULL		induces	NULL				38-kd protein	NULL	phosphorylation of	tyrosine		NULL	HUVECs	0	NULL	NULL	NULL	gw60_amjpathol_159_3_993_s_349	11549592	34  Moreover, the fact that PlGF homodimers that bind to VEGFR-1 and PlGF:VEGF heterodimers that bind to VEGFR-2 induced tyrosine phosphorylation of a 38-kd protein in HUVECs whereas VEGF homodimers did not 29  supports the view that PlGF and VEGF can exert different biological actions through the same receptor.	bind
32422	1	7867	5	13	NULL	NULL	NULL	HSPGs	GP		modulate					FGF-2	GP	signaling of			NULL	human breast cancer	NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_185_s_31	11786412	34  The goal of this project was to investigate HSPGs as modulators of FGF-2 signaling in human breast cancer by addressing the following unresolved questions: 1) Do breast carcinoma HSPGs differ from normal breast epithelial cell HSPGs in their capacity to promote FGF-2 binding to FGFR-1?	bind
32423	2	7867	5	13	NULL	NULL	NULL	FGF-2	GP		bind					FGFR-1	GP				NULL	human breast cancer	NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_185_s_31	11786412	34  The goal of this project was to investigate HSPGs as modulators of FGF-2 signaling in human breast cancer by addressing the following unresolved questions: 1) Do breast carcinoma HSPGs differ from normal breast epithelial cell HSPGs in their capacity to promote FGF-2 binding to FGFR-1?	bind
39445	3	7867	5	13	NULL	NULL	NULL	HSPGs	GP		promotes					statement 2	Process				NULL	human breast cancer	NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_185_s_31	11786412	34  The goal of this project was to investigate HSPGs as modulators of FGF-2 signaling in human breast cancer by addressing the following unresolved questions: 1) Do breast carcinoma HSPGs differ from normal breast epithelial cell HSPGs in their capacity to promote FGF-2 binding to FGFR-1?	bind
25026	1	7867	6	NULL	NULL	0	NULL	FGF-2	NULL		bind	NULL				FGFR-1	NULL				NULL	human breast cancer 	NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_185_s_31	11786412	34  The goal of this project was to investigate HSPGs as modulators of FGF-2 signaling in human breast cancer by addressing the following unresolved questions: 1) Do breast carcinoma HSPGs differ from normal breast epithelial cell HSPGs in their capacity to promote FGF-2 binding to FGFR-1?	bind
25027	2	7867	6	NULL	NULL	0	NULL	HSPG	NULL		promote	NULL				statement 1	NULL				NULL	human breast cancer	NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_185_s_31	11786412	34  The goal of this project was to investigate HSPGs as modulators of FGF-2 signaling in human breast cancer by addressing the following unresolved questions: 1) Do breast carcinoma HSPGs differ from normal breast epithelial cell HSPGs in their capacity to promote FGF-2 binding to FGFR-1?	bind
25028	3	7867	6	NULL	NULL	0	NULL	HSPG	NULL		modulate	NULL				FGF-2	NULL	signaling of			NULL	human breast cancer	NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_185_s_31	11786412	34  The goal of this project was to investigate HSPGs as modulators of FGF-2 signaling in human breast cancer by addressing the following unresolved questions: 1) Do breast carcinoma HSPGs differ from normal breast epithelial cell HSPGs in their capacity to promote FGF-2 binding to FGFR-1?	bind
32425	1	7868	5	13	NULL	NULL	NULL	RAR alpha	GP		is a type of					RA receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
32426	2	7868	5	13	NULL	NULL	NULL	RAR beta	GP		is a type of					RA receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
32427	3	7868	5	13	NULL	NULL	NULL	RAR gamma	GP		is a type of					RA receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
32428	4	7868	5	13	NULL	NULL	NULL	RAR alpha	GP		bind					atRA	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
32429	5	7868	5	13	NULL	NULL	NULL	RAR alpha	GP		bind					9- cis RA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
32430	6	7868	5	13	NULL	NULL	NULL	RAR beta	GP		bind					atRA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
32431	7	7868	5	13	NULL	NULL	NULL	RAR beta	GP		bind					9- cis RA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
32432	8	7868	5	13	NULL	NULL	NULL	RAR gamma	GP		bind					atRA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
32433	9	7868	5	13	NULL	NULL	NULL	RAR gamma	GP		bind					9- cis RA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
32434	10	7868	5	13	NULL	NULL	NULL	RXR alpha	GP		is a type of					retinoid X receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
32435	11	7868	5	13	NULL	NULL	NULL	RXR beta	GP		is a type of					retinoid X receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
32436	12	7868	5	13	NULL	NULL	NULL	RXR gamma	GP		is a type of					retinoid X receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
32438	13	7868	5	13	NULL	NULL	NULL	RXR alpha	GP		bind					9- cis RA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
32439	14	7868	5	13	NULL	NULL	NULL	RXR beta	GP		bind					9- cis RA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
32440	15	7868	5	13	NULL	NULL	NULL	RXR gamma	GP		bind					9- cis RA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
55552	16	7868	5	13	NULL	NULL	NULL	RXR	GP		is					retinoid X receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
25029	1	7868	6	NULL	NULL	0	NULL	RAR alpha	NULL		bind	NULL				atRA	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
25030	2	7868	6	NULL	NULL	0	NULL	RAR beta	NULL		bind	NULL				atRA	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
25031	3	7868	6	NULL	NULL	0	NULL	RAR gamma	NULL		bind	NULL				atRA	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
25032	4	7868	6	NULL	NULL	0	NULL	RAR alpha	NULL		bind	NULL				9- cis RA	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
25033	5	7868	6	NULL	NULL	0	NULL	RAR beta	NULL		bind	NULL				9- cis RA	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
25034	6	7868	6	NULL	NULL	0	NULL	RAR gamma	NULL		bind	NULL				9- cis RA	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
25035	7	7868	6	NULL	NULL	0	NULL	RXR	NULL		is	NULL				retinoid X receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
25036	8	7868	6	NULL	NULL	0	NULL	RXR alpha	NULL		bind	NULL				9- cis RA	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
25037	9	7868	6	NULL	NULL	0	NULL	RXR beta	NULL		bind	NULL				9- cis RA	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
25038	10	7868	6	NULL	NULL	0	NULL	RXR gamma	NULL		bind	NULL				9- cis RA	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
38833	11	7868	6	NULL	NULL	0	NULL	RAR alpha	NULL		is a type of	NULL				RA receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
38834	12	7868	6	NULL	NULL	0	NULL	RAR beta	NULL		is a type of	NULL				RA receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
38835	13	7868	6	NULL	NULL	0	NULL	RAR gamma	NULL		is a type of	NULL				RA receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
38836	14	7868	6	NULL	NULL	0	NULL	RXR alpha	NULL		is a type of	NULL				retinoid X receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
38837	15	7868	6	NULL	NULL	0	NULL	RXR beta	NULL		is a type of	NULL				retinoid X receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
38838	16	7868	6	NULL	NULL	0	NULL	RXR gamma	NULL		is a type of	NULL				retinoid X receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_5_355_s_50	10969032	34  The RA receptors (RARs alpha, beta, and gamma) bind both atRA and 9- cis RA, whereas the retinoid X receptors (RXRs alpha, beta, and gamma) bind 9- cis RA (Figure  ).	bind
32444	1	7869	5	13	NULL	NULL	NULL	apo A-I genes	GP	rabbit	is homologus to		highly			apo A-I genes	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1424_s_154	8977445	34  Therefore, despite a high sequence homology (>78%) of the 200 bp of the 5' upstream flanking region of the rabbit and human apo A-I genes, the nonparenchymal cell - secreted factor that attenuates rabbit hepatic apo A-I gene expression may not bind to this human apo A-I gene fragment.	bind
32526	2	7869	5	13	NULL	NULL	NULL	nonparenchymal cell - secreted factor	GP		attenuates					hepatic apo A-I gene	GP	expression of;; rabbit hepatic			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1424_s_154	8977445	34  Therefore, despite a high sequence homology (>78%) of the 200 bp of the 5' upstream flanking region of the rabbit and human apo A-I genes, the nonparenchymal cell - secreted factor that attenuates rabbit hepatic apo A-I gene expression may not bind to this human apo A-I gene fragment.	bind
32531	3	7869	5	13	NULL	NULL	NULL	nonparenchymal cell - secreted factor	GP		 not bind		may			apo A-I gene fragment	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1424_s_154	8977445	34  Therefore, despite a high sequence homology (>78%) of the 200 bp of the 5' upstream flanking region of the rabbit and human apo A-I genes, the nonparenchymal cell - secreted factor that attenuates rabbit hepatic apo A-I gene expression may not bind to this human apo A-I gene fragment.	bind
25854	1	7869	6	NULL	NULL	0	NULL	apo A-I gene	NULL	rabbit	has homology to	NULL	highly			apo A-I gene	NULL	human			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1424_s_154	8977445	34  Therefore, despite a high sequence homology (>78%) of the 200 bp of the 5' upstream flanking region of the rabbit and human apo A-I genes, the nonparenchymal cell - secreted factor that attenuates rabbit hepatic apo A-I gene expression may not bind to this human apo A-I gene fragment.	bind
25855	2	7869	6	NULL	NULL	0	NULL	nonparenchymal cell - secreted factor	NULL		attenuates	NULL				apo A-I gene	NULL	rabbit;; hepatic;; expression of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1424_s_154	8977445	34  Therefore, despite a high sequence homology (>78%) of the 200 bp of the 5' upstream flanking region of the rabbit and human apo A-I genes, the nonparenchymal cell - secreted factor that attenuates rabbit hepatic apo A-I gene expression may not bind to this human apo A-I gene fragment.	bind
25856	3	7869	6	NULL	NULL	0	NULL	nonparenchymal cell - secreted factor	NULL		not bind	NULL	may			apo A-I gene fragment	NULL	human			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1424_s_154	8977445	34  Therefore, despite a high sequence homology (>78%) of the 200 bp of the 5' upstream flanking region of the rabbit and human apo A-I genes, the nonparenchymal cell - secreted factor that attenuates rabbit hepatic apo A-I gene expression may not bind to this human apo A-I gene fragment.	bind
32441	1	7870	5	13	NULL	NULL	NULL	calcium/calmodulin	GP		bind					eNOS	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1161_s_82	12689915	34 - 36   Optimal eNOS activity occurs when the eNOS/caveolin-1 interaction is competitively disrupted by calcium/calmodulin binding to eNOS.	bind
32442	2	7870	5	13	NULL	NULL	NULL	statement 1	Process		disrupt		competitively			eNOS/caveolin-1	GP	interaction of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1161_s_82	12689915	34 - 36   Optimal eNOS activity occurs when the eNOS/caveolin-1 interaction is competitively disrupted by calcium/calmodulin binding to eNOS.	bind
32443	3	7870	5	13	NULL	NULL	NULL	statement 2	Process		results in					eNOS	GP	optimal activity of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1161_s_82	12689915	34 - 36   Optimal eNOS activity occurs when the eNOS/caveolin-1 interaction is competitively disrupted by calcium/calmodulin binding to eNOS.	bind
25054	1	7870	6	NULL	NULL	0	NULL	calcium/calmodulin	NULL		bind	NULL				eNOS	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1161_s_82	12689915	34 - 36   Optimal eNOS activity occurs when the eNOS/caveolin-1 interaction is competitively disrupted by calcium/calmodulin binding to eNOS.	bind
25057	2	7870	6	NULL	NULL	0	NULL	eNOS/caveolin-1	NULL	interaction of	is disrupted by	NULL	competitively			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1161_s_82	12689915	34 - 36   Optimal eNOS activity occurs when the eNOS/caveolin-1 interaction is competitively disrupted by calcium/calmodulin binding to eNOS.	bind
25059	3	7870	6	10	NULL	0	NULL	statement 2			results in					eNOS		optimal activity of 			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1161_s_82	12689915	34 - 36   Optimal eNOS activity occurs when the eNOS/caveolin-1 interaction is competitively disrupted by calcium/calmodulin binding to eNOS.	bind
32561	1	7871	5	13	NULL	NULL	NULL	LDL	GP		bind					mast cell granules	CellComponent	exocytosed			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_6_801_s_32	7773737	34 35 36  For the present article, we studied whether SMCs, the other potential precursor of foam cells in the arterial intima, would also be capable of taking up LDL bound to exocytosed mast cell granules.	bind
38971	2	7871	5	13	NULL	NULL	NULL	SMC	Cell		precursor of		potentially			foam cells	Cell				NULL	arterial intima	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_6_801_s_32	7773737	34 35 36  For the present article, we studied whether SMCs, the other potential precursor of foam cells in the arterial intima, would also be capable of taking up LDL bound to exocytosed mast cell granules.	bind
25061	1	7871	6	NULL	NULL	0	NULL	SMC	NULL		are precursor of	NULL	potentially			foam cells	NULL				NULL	arterial intima	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_6_801_s_32	7773737	34 35 36  For the present article, we studied whether SMCs, the other potential precursor of foam cells in the arterial intima, would also be capable of taking up LDL bound to exocytosed mast cell granules.	bind
25064	2	7871	6	NULL	NULL	0	NULL	LDL	NULL		bind	NULL				mast cell granules	NULL	exocytosed			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_6_801_s_32	7773737	34 35 36  For the present article, we studied whether SMCs, the other potential precursor of foam cells in the arterial intima, would also be capable of taking up LDL bound to exocytosed mast cell granules.	bind
32562	1	7872	5	13	NULL	NULL	NULL	CREB	GP		is					CRE binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_68	15681294	34 A large number of transactivators including CRE binding protein (CREB), ATF, C/EBP, C-Jun, C-Fos, and USF bind to an overlapped CRE and AP-1 region located at  - 60 to  - 40 from the transcription start site.	bind
32563	2	7872	5	13	NULL	NULL	NULL	CREB	GP		is a type of					transactivator	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_68	15681294	34 A large number of transactivators including CRE binding protein (CREB), ATF, C/EBP, C-Jun, C-Fos, and USF bind to an overlapped CRE and AP-1 region located at  - 60 to  - 40 from the transcription start site.	bind
32564	3	7872	5	13	NULL	NULL	NULL	ATF	GP		is a type of					transactivator	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_68	15681294	34 A large number of transactivators including CRE binding protein (CREB), ATF, C/EBP, C-Jun, C-Fos, and USF bind to an overlapped CRE and AP-1 region located at  - 60 to  - 40 from the transcription start site.	bind
32565	4	7872	5	13	NULL	NULL	NULL	C/EBP	GP		is a type of					transactivator	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_68	15681294	34 A large number of transactivators including CRE binding protein (CREB), ATF, C/EBP, C-Jun, C-Fos, and USF bind to an overlapped CRE and AP-1 region located at  - 60 to  - 40 from the transcription start site.	bind
32566	5	7872	5	13	NULL	NULL	NULL	C-Jun	GP		is a type of					transactivator	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_68	15681294	34 A large number of transactivators including CRE binding protein (CREB), ATF, C/EBP, C-Jun, C-Fos, and USF bind to an overlapped CRE and AP-1 region located at  - 60 to  - 40 from the transcription start site.	bind
32567	6	7872	5	13	NULL	NULL	NULL	C-Fos	GP		is a type of					transactivator	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_68	15681294	34 A large number of transactivators including CRE binding protein (CREB), ATF, C/EBP, C-Jun, C-Fos, and USF bind to an overlapped CRE and AP-1 region located at  - 60 to  - 40 from the transcription start site.	bind
32568	7	7872	5	13	NULL	NULL	NULL	USF	GP		is a type of					transactivator	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_68	15681294	34 A large number of transactivators including CRE binding protein (CREB), ATF, C/EBP, C-Jun, C-Fos, and USF bind to an overlapped CRE and AP-1 region located at  - 60 to  - 40 from the transcription start site.	bind
32569	8	7872	5	NULL	NULL	0	NULL		NULL	overlapped	is located at	NULL			CRE;;AP-1 region		NULL			 - 60 to - 40 from transcription start site	NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_68	15681294	34 A large number of transactivators including CRE binding protein (CREB), ATF, C/EBP, C-Jun, C-Fos, and USF bind to an overlapped CRE and AP-1 region located at  - 60 to  - 40 from the transcription start site.	bind
32787	9	7872	5	13	NULL	NULL	NULL	CREB	GP		bind					statement 15	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_68	15681294	34 A large number of transactivators including CRE binding protein (CREB), ATF, C/EBP, C-Jun, C-Fos, and USF bind to an overlapped CRE and AP-1 region located at  - 60 to  - 40 from the transcription start site.	bind
32788	10	7872	5	13	NULL	NULL	NULL	ATF	GP		bind					statement 15	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_68	15681294	34 A large number of transactivators including CRE binding protein (CREB), ATF, C/EBP, C-Jun, C-Fos, and USF bind to an overlapped CRE and AP-1 region located at  - 60 to  - 40 from the transcription start site.	bind
32789	11	7872	5	13	NULL	NULL	NULL	C/EBP	GP		bind					statement 15	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_68	15681294	34 A large number of transactivators including CRE binding protein (CREB), ATF, C/EBP, C-Jun, C-Fos, and USF bind to an overlapped CRE and AP-1 region located at  - 60 to  - 40 from the transcription start site.	bind
32791	12	7872	5	13	NULL	NULL	NULL	C-Jun	GP		bind					statement 15	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_68	15681294	34 A large number of transactivators including CRE binding protein (CREB), ATF, C/EBP, C-Jun, C-Fos, and USF bind to an overlapped CRE and AP-1 region located at  - 60 to  - 40 from the transcription start site.	bind
32792	13	7872	5	13	NULL	NULL	NULL	C-Fos	GP		bind					statement 15	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_68	15681294	34 A large number of transactivators including CRE binding protein (CREB), ATF, C/EBP, C-Jun, C-Fos, and USF bind to an overlapped CRE and AP-1 region located at  - 60 to  - 40 from the transcription start site.	bind
32793	14	7872	5	13	NULL	NULL	NULL	USF	GP		bind					statement 15	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_68	15681294	34 A large number of transactivators including CRE binding protein (CREB), ATF, C/EBP, C-Jun, C-Fos, and USF bind to an overlapped CRE and AP-1 region located at  - 60 to  - 40 from the transcription start site.	bind
55553	15	7872	5	10	NULL	0	NULL				overlaps				CRE					AP-1 region	NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_68	15681294	34 A large number of transactivators including CRE binding protein (CREB), ATF, C/EBP, C-Jun, C-Fos, and USF bind to an overlapped CRE and AP-1 region located at  - 60 to  - 40 from the transcription start site.	bind
25074	1	7872	6	NULL	NULL	0	NULL	CREB	NULL		is	NULL				CRE binding protein	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_68	15681294	34 A large number of transactivators including CRE binding protein (CREB), ATF, C/EBP, C-Jun, C-Fos, and USF bind to an overlapped CRE and AP-1 region located at  - 60 to  - 40 from the transcription start site.	bind
25076	2	7872	6	10	NULL	0	NULL				overlaps with				CRE	AP-1 region					NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_68	15681294	34 A large number of transactivators including CRE binding protein (CREB), ATF, C/EBP, C-Jun, C-Fos, and USF bind to an overlapped CRE and AP-1 region located at  - 60 to  - 40 from the transcription start site.	bind
25079	3	7872	6	NULL	NULL	0	NULL	statement 2	NULL		is located at	NULL					NULL			- 60 to - 40 from the transcription start site	NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_68	15681294	34 A large number of transactivators including CRE binding protein (CREB), ATF, C/EBP, C-Jun, C-Fos, and USF bind to an overlapped CRE and AP-1 region located at  - 60 to  - 40 from the transcription start site.	bind
25082	4	7872	6	NULL	NULL	0	NULL	CREB	NULL		bind	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_68	15681294	34 A large number of transactivators including CRE binding protein (CREB), ATF, C/EBP, C-Jun, C-Fos, and USF bind to an overlapped CRE and AP-1 region located at  - 60 to  - 40 from the transcription start site.	bind
25083	5	7872	6	NULL	NULL	0	NULL	ATF	NULL		bind	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_68	15681294	34 A large number of transactivators including CRE binding protein (CREB), ATF, C/EBP, C-Jun, C-Fos, and USF bind to an overlapped CRE and AP-1 region located at  - 60 to  - 40 from the transcription start site.	bind
25084	6	7872	6	NULL	NULL	0	NULL	C/EBP	NULL		bind	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_68	15681294	34 A large number of transactivators including CRE binding protein (CREB), ATF, C/EBP, C-Jun, C-Fos, and USF bind to an overlapped CRE and AP-1 region located at  - 60 to  - 40 from the transcription start site.	bind
25085	7	7872	6	NULL	NULL	0	NULL	C-jun	NULL		bind	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_68	15681294	34 A large number of transactivators including CRE binding protein (CREB), ATF, C/EBP, C-Jun, C-Fos, and USF bind to an overlapped CRE and AP-1 region located at  - 60 to  - 40 from the transcription start site.	bind
25086	8	7872	6	NULL	NULL	0	NULL	C-Fos	NULL		bind	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_68	15681294	34 A large number of transactivators including CRE binding protein (CREB), ATF, C/EBP, C-Jun, C-Fos, and USF bind to an overlapped CRE and AP-1 region located at  - 60 to  - 40 from the transcription start site.	bind
25087	9	7872	6	NULL	NULL	0	NULL	USF	NULL		bind	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_68	15681294	34 A large number of transactivators including CRE binding protein (CREB), ATF, C/EBP, C-Jun, C-Fos, and USF bind to an overlapped CRE and AP-1 region located at  - 60 to  - 40 from the transcription start site.	bind
38839	10	7872	6	NULL	NULL	0	NULL	CREB	NULL		is a type of	NULL				transactivator	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_68	15681294	34 A large number of transactivators including CRE binding protein (CREB), ATF, C/EBP, C-Jun, C-Fos, and USF bind to an overlapped CRE and AP-1 region located at  - 60 to  - 40 from the transcription start site.	bind
38840	11	7872	6	NULL	NULL	0	NULL	ATF	NULL		is a type of	NULL				transactivator	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_68	15681294	34 A large number of transactivators including CRE binding protein (CREB), ATF, C/EBP, C-Jun, C-Fos, and USF bind to an overlapped CRE and AP-1 region located at  - 60 to  - 40 from the transcription start site.	bind
38841	12	7872	6	NULL	NULL	0	NULL	C/EBP	NULL		is a type of	NULL				transactivator	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_68	15681294	34 A large number of transactivators including CRE binding protein (CREB), ATF, C/EBP, C-Jun, C-Fos, and USF bind to an overlapped CRE and AP-1 region located at  - 60 to  - 40 from the transcription start site.	bind
38842	13	7872	6	NULL	NULL	0	NULL	C-jun	NULL		is a type of	NULL				transactivator	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_68	15681294	34 A large number of transactivators including CRE binding protein (CREB), ATF, C/EBP, C-Jun, C-Fos, and USF bind to an overlapped CRE and AP-1 region located at  - 60 to  - 40 from the transcription start site.	bind
38843	14	7872	6	NULL	NULL	0	NULL	C-fos	NULL		is a type of	NULL				transactivator	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_68	15681294	34 A large number of transactivators including CRE binding protein (CREB), ATF, C/EBP, C-Jun, C-Fos, and USF bind to an overlapped CRE and AP-1 region located at  - 60 to  - 40 from the transcription start site.	bind
38844	15	7872	6	NULL	NULL	0	NULL	USF	NULL		is a type of	NULL				transactivator	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_68	15681294	34 A large number of transactivators including CRE binding protein (CREB), ATF, C/EBP, C-Jun, C-Fos, and USF bind to an overlapped CRE and AP-1 region located at  - 60 to  - 40 from the transcription start site.	bind
32532	1	7873	5	13	NULL	NULL	NULL	FGF2	GP		bind					HSPG	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_316_s_226	14684627	34 Alternatively, the binding of FGF2 to HSPG could facilitate the interaction of the heparan sulfate chains with heparin receptors on the cell, which have been demonstrated to lead to ERK1/2 activation in VSMCs. 35	bind
32538	2	7873	5	13	NULL	NULL	NULL	heparan sulfate chains	Chemical		interacts with					heparin receptors	GP				NULL	on cell	NULL	NULL	NULL	NULL	gw70_circulationres_94_3_316_s_226	14684627	34 Alternatively, the binding of FGF2 to HSPG could facilitate the interaction of the heparan sulfate chains with heparin receptors on the cell, which have been demonstrated to lead to ERK1/2 activation in VSMCs. 35	bind
32539	3	7873	5	13	NULL	NULL	NULL	statement 1	Process		facilitate					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_316_s_226	14684627	34 Alternatively, the binding of FGF2 to HSPG could facilitate the interaction of the heparan sulfate chains with heparin receptors on the cell, which have been demonstrated to lead to ERK1/2 activation in VSMCs. 35	bind
32540	4	7873	5	13	NULL	NULL	NULL	statement 2	Process		leads to					ERK1/2	GP	activation of			NULL	VSMCs	NULL	NULL	NULL	NULL	gw70_circulationres_94_3_316_s_226	14684627	34 Alternatively, the binding of FGF2 to HSPG could facilitate the interaction of the heparan sulfate chains with heparin receptors on the cell, which have been demonstrated to lead to ERK1/2 activation in VSMCs. 35	bind
25088	1	7873	6	NULL	NULL	0	NULL	FGF2	NULL		bind	NULL				HSPG	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_3_316_s_226	14684627	34 Alternatively, the binding of FGF2 to HSPG could facilitate the interaction of the heparan sulfate chains with heparin receptors on the cell, which have been demonstrated to lead to ERK1/2 activation in VSMCs. 35	bind
25089	2	7873	6	NULL	NULL	0	NULL	heparan sulfate chains	NULL		interacts with	NULL				heparin receptors	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_3_316_s_226	14684627	34 Alternatively, the binding of FGF2 to HSPG could facilitate the interaction of the heparan sulfate chains with heparin receptors on the cell, which have been demonstrated to lead to ERK1/2 activation in VSMCs. 35	bind
25090	3	7873	6	NULL	NULL	0	NULL	statement 1	NULL		facilitate	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_3_316_s_226	14684627	34 Alternatively, the binding of FGF2 to HSPG could facilitate the interaction of the heparan sulfate chains with heparin receptors on the cell, which have been demonstrated to lead to ERK1/2 activation in VSMCs. 35	bind
25091	4	7873	6	NULL	NULL	0	NULL	statement 3	NULL		lead to	NULL				ERK1/2	NULL	activation of			NULL	VSMCs	0	NULL	NULL	NULL	gw70_circulationres_94_3_316_s_226	14684627	34 Alternatively, the binding of FGF2 to HSPG could facilitate the interaction of the heparan sulfate chains with heparin receptors on the cell, which have been demonstrated to lead to ERK1/2 activation in VSMCs. 35	bind
32541	1	7874	5	13	NULL	NULL	NULL	CRP	GP		does not bind					ECs	Cell	healthy;; cultured			NULL	in vitro in cultured vascular cells	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1225_s_157	15802626	34 In the in vitro investigations using cultured vascular cells, the initiating step of CRP binding to healthy cultured ECs has simply not been met, which explains the absence of any effect of CRP in our in vitro studies.	bind
25138	1	7874	6	10	NULL	0	NULL	CRP	NULL		does not bind	NULL				EC	NULL	healthy;;cultured			NULL	in vitro in cultured vascular cells	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1225_s_157	15802626	34 In the in vitro investigations using cultured vascular cells, the initiating step of CRP binding to healthy cultured ECs has simply not been met, which explains the absence of any effect of CRP in our in vitro studies.	bind
32543	1	7875	5	13	NULL	NULL	NULL	ABCA1	GP		bind					apoA-I	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_58	12738681	34 Like scavenger receptor BI, ABCA1 binds not only apoA-I but also other apolipoproteins, including apoE. 35 Thus, the antiatherogenic effect of apoE in vivo could be partially explained by lipid efflux from macrophage foam cells coordinated with ABCA1.	bind
32544	2	7875	5	13	NULL	NULL	NULL	ABCA1	GP		bind					apoE	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_58	12738681	34 Like scavenger receptor BI, ABCA1 binds not only apoA-I but also other apolipoproteins, including apoE. 35 Thus, the antiatherogenic effect of apoE in vivo could be partially explained by lipid efflux from macrophage foam cells coordinated with ABCA1.	bind
32545	3	7875	5	13	NULL	NULL	NULL	apoE	GP		is a type of					apolipoproteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_58	12738681	34 Like scavenger receptor BI, ABCA1 binds not only apoA-I but also other apolipoproteins, including apoE. 35 Thus, the antiatherogenic effect of apoE in vivo could be partially explained by lipid efflux from macrophage foam cells coordinated with ABCA1.	bind
32547	4	7875	5	13	NULL	NULL	NULL	 BI	GP		bind					apoA-I	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_58	12738681	34 Like scavenger receptor BI, ABCA1 binds not only apoA-I but also other apolipoproteins, including apoE. 35 Thus, the antiatherogenic effect of apoE in vivo could be partially explained by lipid efflux from macrophage foam cells coordinated with ABCA1.	bind
32549	5	7875	5	13	NULL	NULL	NULL	 BI	GP		bind					apoE	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_58	12738681	34 Like scavenger receptor BI, ABCA1 binds not only apoA-I but also other apolipoproteins, including apoE. 35 Thus, the antiatherogenic effect of apoE in vivo could be partially explained by lipid efflux from macrophage foam cells coordinated with ABCA1.	bind
32554	6	7875	5	13	NULL	NULL	NULL	lipid efflux	Process	macrophage foam cells	coordinate with					ABCA1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_58	12738681	34 Like scavenger receptor BI, ABCA1 binds not only apoA-I but also other apolipoproteins, including apoE. 35 Thus, the antiatherogenic effect of apoE in vivo could be partially explained by lipid efflux from macrophage foam cells coordinated with ABCA1.	bind
32555	7	7875	5	13	NULL	NULL	NULL	statement 6	Process		explains		partially			apoE	GP	antiatherogenic effect of 			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_58	12738681	34 Like scavenger receptor BI, ABCA1 binds not only apoA-I but also other apolipoproteins, including apoE. 35 Thus, the antiatherogenic effect of apoE in vivo could be partially explained by lipid efflux from macrophage foam cells coordinated with ABCA1.	bind
47547	8	7875	5	13	NULL	NULL	NULL	BI	GP		is a type of					scavenger receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_58	12738681	34 Like scavenger receptor BI, ABCA1 binds not only apoA-I but also other apolipoproteins, including apoE. 35 Thus, the antiatherogenic effect of apoE in vivo could be partially explained by lipid efflux from macrophage foam cells coordinated with ABCA1.	bind
25139	1	7875	6	NULL	NULL	0	NULL	ABCA1	NULL		bind	NULL				apoA-I	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_58	12738681	34 Like scavenger receptor BI, ABCA1 binds not only apoA-I but also other apolipoproteins, including apoE. 35 Thus, the antiatherogenic effect of apoE in vivo could be partially explained by lipid efflux from macrophage foam cells coordinated with ABCA1.	bind
25140	2	7875	6	NULL	NULL	0	NULL	ABCA1	NULL		bind	NULL				apoE	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_58	12738681	34 Like scavenger receptor BI, ABCA1 binds not only apoA-I but also other apolipoproteins, including apoE. 35 Thus, the antiatherogenic effect of apoE in vivo could be partially explained by lipid efflux from macrophage foam cells coordinated with ABCA1.	bind
25141	3	7875	6	NULL	NULL	0	NULL	scavenger receptor BI	NULL		bind	NULL				apoA-I	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_58	12738681	34 Like scavenger receptor BI, ABCA1 binds not only apoA-I but also other apolipoproteins, including apoE. 35 Thus, the antiatherogenic effect of apoE in vivo could be partially explained by lipid efflux from macrophage foam cells coordinated with ABCA1.	bind
25142	4	7875	6	NULL	NULL	0	NULL	scavenger receptor BI	NULL		bind	NULL				apoE	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_58	12738681	34 Like scavenger receptor BI, ABCA1 binds not only apoA-I but also other apolipoproteins, including apoE. 35 Thus, the antiatherogenic effect of apoE in vivo could be partially explained by lipid efflux from macrophage foam cells coordinated with ABCA1.	bind
25848	6	7875	6	NULL	NULL	0	NULL	macrophage foam cells	NULL		exhibits	NULL				lipid efflux	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_58	12738681	34 Like scavenger receptor BI, ABCA1 binds not only apoA-I but also other apolipoproteins, including apoE. 35 Thus, the antiatherogenic effect of apoE in vivo could be partially explained by lipid efflux from macrophage foam cells coordinated with ABCA1.	bind
25849	7	7875	6	NULL	NULL	0	NULL	statement 6	NULL		is coordinated with	NULL				ABCA1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_58	12738681	34 Like scavenger receptor BI, ABCA1 binds not only apoA-I but also other apolipoproteins, including apoE. 35 Thus, the antiatherogenic effect of apoE in vivo could be partially explained by lipid efflux from macrophage foam cells coordinated with ABCA1.	bind
25850	8	7875	6	10	NULL	0	NULL	statement 5			because of		may			apoE		antiatherogenic effect of 			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_58	12738681	34 Like scavenger receptor BI, ABCA1 binds not only apoA-I but also other apolipoproteins, including apoE. 35 Thus, the antiatherogenic effect of apoE in vivo could be partially explained by lipid efflux from macrophage foam cells coordinated with ABCA1.	bind
47548	9	7875	6	10	NULL	0	NULL	BI	NULL		is a type of	NULL				scavenger receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_58	12738681	34 Like scavenger receptor BI, ABCA1 binds not only apoA-I but also other apolipoproteins, including apoE. 35 Thus, the antiatherogenic effect of apoE in vivo could be partially explained by lipid efflux from macrophage foam cells coordinated with ABCA1.	bind
32556	1	7876	5	13	NULL	NULL	NULL	MyBP-C	GP		bind					myosin	GP		S2 portion		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_89_12_1184_s_166	11739284	34 Phosphorylation of MyBP-C has been reported to relieve the binding of the MyBP-C to the S2 portion of myosin, 35 which may allow greater crossbridge extension from the thick filament and alter crossbridge orientation.	bind
32557	2	7876	5	13	NULL	NULL	NULL	MyBP-C	GP	phosphorylation of	relieve					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_89_12_1184_s_166	11739284	34 Phosphorylation of MyBP-C has been reported to relieve the binding of the MyBP-C to the S2 portion of myosin, 35 which may allow greater crossbridge extension from the thick filament and alter crossbridge orientation.	bind
32558	3	7876	5	13	NULL	NULL	NULL	statement 2	Process		allows					crossbridge extension	Process	greater			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_89_12_1184_s_166	11739284	34 Phosphorylation of MyBP-C has been reported to relieve the binding of the MyBP-C to the S2 portion of myosin, 35 which may allow greater crossbridge extension from the thick filament and alter crossbridge orientation.	bind
32560	4	7876	5	13	NULL	NULL	NULL	statement 2	Process		alters					crossbridge orientation	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_89_12_1184_s_166	11739284	34 Phosphorylation of MyBP-C has been reported to relieve the binding of the MyBP-C to the S2 portion of myosin, 35 which may allow greater crossbridge extension from the thick filament and alter crossbridge orientation.	bind
25143	1	7876	6	NULL	NULL	0	NULL	MyBP-C	NULL		bind	NULL				myosin	NULL		S2 portion		NULL		0	NULL	NULL	NULL	gw60_circulationres_89_12_1184_s_166	11739284	34 Phosphorylation of MyBP-C has been reported to relieve the binding of the MyBP-C to the S2 portion of myosin, 35 which may allow greater crossbridge extension from the thick filament and alter crossbridge orientation.	bind
25144	2	7876	6	NULL	NULL	0	NULL	MyBP-C	NULL	phosphorylation of	relieves	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_89_12_1184_s_166	11739284	34 Phosphorylation of MyBP-C has been reported to relieve the binding of the MyBP-C to the S2 portion of myosin, 35 which may allow greater crossbridge extension from the thick filament and alter crossbridge orientation.	bind
25258	3	7876	6	NULL	NULL	0	NULL	statement 2	NULL		allow	NULL	may			crossbridge extension	NULL	greater			NULL		0	NULL	NULL	NULL	gw60_circulationres_89_12_1184_s_166	11739284	34 Phosphorylation of MyBP-C has been reported to relieve the binding of the MyBP-C to the S2 portion of myosin, 35 which may allow greater crossbridge extension from the thick filament and alter crossbridge orientation.	bind
25259	4	7876	6	NULL	NULL	0	NULL	statement 2	NULL		alter	NULL				crossbridge orientation	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_89_12_1184_s_166	11739284	34 Phosphorylation of MyBP-C has been reported to relieve the binding of the MyBP-C to the S2 portion of myosin, 35 which may allow greater crossbridge extension from the thick filament and alter crossbridge orientation.	bind
32794	1	7877	5	13	NULL	NULL	NULL	Sp1	GP		bind					PKG-Ialpha	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_4_405_s_226	11884369	34, 35 Our data show that a decrease in Sp1 binding activity to the PKG-Ialpha promoter by cyclic nucleotide analogues are dependent on activation of PKA consistent with the role of phosphorylation in modifying Sp1 binding activity.	bind
32795	2	7877	5	13	NULL	NULL	NULL	cyclic nucleotide analogues	Chemical		decrease					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_4_405_s_226	11884369	34, 35 Our data show that a decrease in Sp1 binding activity to the PKG-Ialpha promoter by cyclic nucleotide analogues are dependent on activation of PKA consistent with the role of phosphorylation in modifying Sp1 binding activity.	bind
32796	3	7877	5	13	NULL	NULL	NULL	statement 2	Process		is dependent on					PKA	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_4_405_s_226	11884369	34, 35 Our data show that a decrease in Sp1 binding activity to the PKG-Ialpha promoter by cyclic nucleotide analogues are dependent on activation of PKA consistent with the role of phosphorylation in modifying Sp1 binding activity.	bind
32797	4	7877	5	13	NULL	NULL	NULL	phosphorylation	Process		modify					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_4_405_s_226	11884369	34, 35 Our data show that a decrease in Sp1 binding activity to the PKG-Ialpha promoter by cyclic nucleotide analogues are dependent on activation of PKA consistent with the role of phosphorylation in modifying Sp1 binding activity.	bind
32798	5	7877	5	13	NULL	NULL	NULL	statement 3	Process		consistent with					statement 4	Process	role of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_4_405_s_226	11884369	34, 35 Our data show that a decrease in Sp1 binding activity to the PKG-Ialpha promoter by cyclic nucleotide analogues are dependent on activation of PKA consistent with the role of phosphorylation in modifying Sp1 binding activity.	bind
25260	1	7877	6	NULL	NULL	0	NULL	Sp1	NULL		bind	NULL				PKG-Ialpha	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_circulationres_90_4_405_s_226	11884369	34, 35 Our data show that a decrease in Sp1 binding activity to the PKG-Ialpha promoter by cyclic nucleotide analogues are dependent on activation of PKA consistent with the role of phosphorylation in modifying Sp1 binding activity.	bind
25261	2	7877	6	NULL	NULL	0	NULL	cyclic nucleotide analogues	NULL		decrease	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_4_405_s_226	11884369	34, 35 Our data show that a decrease in Sp1 binding activity to the PKG-Ialpha promoter by cyclic nucleotide analogues are dependent on activation of PKA consistent with the role of phosphorylation in modifying Sp1 binding activity.	bind
25262	3	7877	6	NULL	NULL	0	NULL	statement 2	NULL		is dependent on	NULL				PKA	NULL	activation of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_4_405_s_226	11884369	34, 35 Our data show that a decrease in Sp1 binding activity to the PKG-Ialpha promoter by cyclic nucleotide analogues are dependent on activation of PKA consistent with the role of phosphorylation in modifying Sp1 binding activity.	bind
25263	4	7877	6	NULL	NULL	0	NULL	phosphorylation	NULL		modifies	NULL				statement 1	NULL	binding activity of 			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_4_405_s_226	11884369	34, 35 Our data show that a decrease in Sp1 binding activity to the PKG-Ialpha promoter by cyclic nucleotide analogues are dependent on activation of PKA consistent with the role of phosphorylation in modifying Sp1 binding activity.	bind
38845	5	7877	6	10	NULL	0	NULL	statement 3	NULL		consistent with 	NULL				statement 4	NULL	role of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_4_405_s_226	11884369	34, 35 Our data show that a decrease in Sp1 binding activity to the PKG-Ialpha promoter by cyclic nucleotide analogues are dependent on activation of PKA consistent with the role of phosphorylation in modifying Sp1 binding activity.	bind
32799	1	7878	5	13	NULL	NULL	NULL	TIMP-1	GP		bind					MMP-9	GP	inactive			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1837_s_211	9327785	34,50 Therefore, the expression of TIMP-1, which binds to the inactive form of MMP-9, was examined.	bind
25264	1	7878	6	NULL	NULL	0	NULL	TIMP-1	NULL		bind	NULL				MMP-9	NULL	inactive			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1837_s_211	9327785	34,50 Therefore, the expression of TIMP-1, which binds to the inactive form of MMP-9, was examined.	bind
32800	1	7879	5	13	NULL	NULL	NULL	YY1	GP		is a type of					ubiquitous nuclear transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_21_4493_s_371	11691937	35       Becker,K.G., Swergold,G.D., Ozato,K. and Thayer,R.E. (1993) Binding of the ubiquitous nuclear transcription factor YY1 to a  cis regulatory sequence in the human LINE-1 transposable element.	bind
32801	3	7879	5	13	NULL	NULL	NULL	YY1	GP		bind					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_21_4493_s_371	11691937	35       Becker,K.G., Swergold,G.D., Ozato,K. and Thayer,R.E. (1993) Binding of the ubiquitous nuclear transcription factor YY1 to a  cis regulatory sequence in the human LINE-1 transposable element.	bind
55567	2	7879	5	10	NULL	0	NULL	resides in		human					cis regulatory sequence			human		LINE-1 transposable element	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_21_4493_s_371	11691937	35       Becker,K.G., Swergold,G.D., Ozato,K. and Thayer,R.E. (1993) Binding of the ubiquitous nuclear transcription factor YY1 to a  cis regulatory sequence in the human LINE-1 transposable element.	bind
25265	2	7879	6	10	NULL	0	NULL	YY1			bind					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_21_4493_s_371	11691937	35       Becker,K.G., Swergold,G.D., Ozato,K. and Thayer,R.E. (1993) Binding of the ubiquitous nuclear transcription factor YY1 to a  cis regulatory sequence in the human LINE-1 transposable element.	bind
38846	2	7879	6	NULL	NULL	0	NULL	YY1	NULL		is a type of	NULL				ubiquitous nuclear transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_21_4493_s_371	11691937	35       Becker,K.G., Swergold,G.D., Ozato,K. and Thayer,R.E. (1993) Binding of the ubiquitous nuclear transcription factor YY1 to a  cis regulatory sequence in the human LINE-1 transposable element.	bind
55568	1	7879	6	10	NULL	0	NULL			human	resides in				cis regulatory sequence			human		LINE-1 transposable element	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_21_4493_s_371	11691937	35       Becker,K.G., Swergold,G.D., Ozato,K. and Thayer,R.E. (1993) Binding of the ubiquitous nuclear transcription factor YY1 to a  cis regulatory sequence in the human LINE-1 transposable element.	bind
32802	1	7880	5	13	NULL	NULL	NULL	renin	GP	porcine	bind		high affinity			cardiac membranes	OrganismPart	porcine			NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_1_220_s_148	9236437	35  36  In the present study, we observed high-affinity binding of porcine renin to porcine cardiac membranes.	bind
25266	1	7880	6	NULL	NULL	0	NULL	renin	NULL	porcine	bind	NULL	high affinity			cardiac membranes	NULL	porcine			NULL		0	NULL	NULL	NULL	gw60_circulation_96_1_220_s_148	9236437	35  36  In the present study, we observed high-affinity binding of porcine renin to porcine cardiac membranes.	bind
32803	1	7881	5	13	NULL	NULL	NULL	apoB	GP		bind					MBP 200	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_968_s_140	9633939	35  Further, it suggests that the domain in apoB that binds to MBP 200, 235 is not in a heparin-binding domain of apoB.	bind
32804	2	7881	5	13	NULL	NULL	NULL	apoB	GP		bind					MBP 235	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_968_s_140	9633939	35  Further, it suggests that the domain in apoB that binds to MBP 200, 235 is not in a heparin-binding domain of apoB.	bind
32805	3	7881	5	13	NULL	NULL	NULL	apoB	GP		does not bind			heparin-binding domain		MBP 200	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_968_s_140	9633939	35  Further, it suggests that the domain in apoB that binds to MBP 200, 235 is not in a heparin-binding domain of apoB.	bind
32806	4	7881	5	13	NULL	NULL	NULL	apoB	GP		does not bind			heparin-binding domain		MBP 235	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_968_s_140	9633939	35  Further, it suggests that the domain in apoB that binds to MBP 200, 235 is not in a heparin-binding domain of apoB.	bind
25267	1	7881	6	NULL	NULL	0	NULL	apoB	NULL		bind	NULL				MBP 200	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_968_s_140	9633939	35  Further, it suggests that the domain in apoB that binds to MBP 200, 235 is not in a heparin-binding domain of apoB.	bind
25268	2	7881	6	10	NULL	0	NULL	apoB	NULL		bind	NULL				MBP 235	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_968_s_140	9633939	35  Further, it suggests that the domain in apoB that binds to MBP 200, 235 is not in a heparin-binding domain of apoB.	bind
38860	3	7881	6	NULL	NULL	0	NULL	apoB	NULL		does not bind	NULL		heparin binding domain		MBP 200	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_968_s_140	9633939	35  Further, it suggests that the domain in apoB that binds to MBP 200, 235 is not in a heparin-binding domain of apoB.	bind
38861	4	7881	6	NULL	NULL	0	NULL	apoB	NULL		does not bind	NULL		heparin binding domain		MBP 235	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_968_s_140	9633939	35  Further, it suggests that the domain in apoB that binds to MBP 200, 235 is not in a heparin-binding domain of apoB.	bind
32807	1	7882	5	13	NULL	NULL	NULL	Fos-Jun heterodimers	GP		bind					TF	GP			AP-1 sites in enhancer	NULL	in stimulated endothelial cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_5_612_s_234	7749875	35  Here, we showed that in stimulated endothelial cells, Fos-Jun heterodimers bound to the two AP-1 sites and c-Rel - p65 heterodimers bound to an adjacent kappaB-like site in the 56-bp TF enhancer.	bind
32808	2	7882	5	13	NULL	NULL	NULL	c-Rel - p65 heterodimers	GP		bind					TF	GP			adjacent kappaB-like site in enhancer	NULL	in stimulated endothelial cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_5_612_s_234	7749875	35  Here, we showed that in stimulated endothelial cells, Fos-Jun heterodimers bound to the two AP-1 sites and c-Rel - p65 heterodimers bound to an adjacent kappaB-like site in the 56-bp TF enhancer.	bind
25269	1	7882	6	NULL	NULL	0	NULL	Fos-Jun heterodimers	NULL		bind	NULL				TF	NULL			AP-1 site of enhancer	NULL	stimulated endothelial cells	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_5_612_s_234	7749875	35  Here, we showed that in stimulated endothelial cells, Fos-Jun heterodimers bound to the two AP-1 sites and c-Rel - p65 heterodimers bound to an adjacent kappaB-like site in the 56-bp TF enhancer.	bind
25270	2	7882	6	NULL	NULL	0	NULL	c-Rel - p65 heterodimers	NULL		bind	NULL				TF	NULL			kappaB-like site of enhancer	NULL	stimulated endothelial cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_5_612_s_234	7749875	35  Here, we showed that in stimulated endothelial cells, Fos-Jun heterodimers bound to the two AP-1 sites and c-Rel - p65 heterodimers bound to an adjacent kappaB-like site in the 56-bp TF enhancer.	bind
32809	1	7883	5	13	NULL	NULL	NULL	IGF-BP3	GP		bind					IGFs	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_5_1535_s_115	12414501	35  IGF-BP3 binds the IGFs and prevents the activation of the IGF-1 receptor, which normally mediates cell signals to promote myogenesis.	bind
32810	2	7883	5	13	NULL	NULL	NULL	statement 1	Process		prevents					IGF-1 receptor	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_5_1535_s_115	12414501	35  IGF-BP3 binds the IGFs and prevents the activation of the IGF-1 receptor, which normally mediates cell signals to promote myogenesis.	bind
32811	3	7883	5	13	NULL	NULL	NULL	IGF-1 receptor	GP		promote					myogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_5_1535_s_115	12414501	35  IGF-BP3 binds the IGFs and prevents the activation of the IGF-1 receptor, which normally mediates cell signals to promote myogenesis.	bind
32812	5	7883	5	13	NULL	NULL	NULL	statement 3	Process		via					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_5_1535_s_115	12414501	35  IGF-BP3 binds the IGFs and prevents the activation of the IGF-1 receptor, which normally mediates cell signals to promote myogenesis.	bind
38972	4	7883	5	13	NULL	NULL	NULL	IGF-1 receptor	GP		mediate					cell signals	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_5_1535_s_115	12414501	35  IGF-BP3 binds the IGFs and prevents the activation of the IGF-1 receptor, which normally mediates cell signals to promote myogenesis.	bind
25271	1	7883	6	NULL	NULL	0	NULL	IGF-BP3	NULL		bind	NULL				IGF	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_5_1535_s_115	12414501	35  IGF-BP3 binds the IGFs and prevents the activation of the IGF-1 receptor, which normally mediates cell signals to promote myogenesis.	bind
25272	2	7883	6	NULL	NULL	0	NULL	statement 1	NULL		prevent	NULL				IGF-1 receptor	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_5_1535_s_115	12414501	35  IGF-BP3 binds the IGFs and prevents the activation of the IGF-1 receptor, which normally mediates cell signals to promote myogenesis.	bind
25273	3	7883	6	NULL	NULL	0	NULL	IGF-1 receptor	NULL		promotes	NULL				myogenesis	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_5_1535_s_115	12414501	35  IGF-BP3 binds the IGFs and prevents the activation of the IGF-1 receptor, which normally mediates cell signals to promote myogenesis.	bind
25274	4	7883	6	NULL	NULL	0	NULL	IGF-1 receptor	NULL		mediates	NULL				cell signals	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_5_1535_s_115	12414501	35  IGF-BP3 binds the IGFs and prevents the activation of the IGF-1 receptor, which normally mediates cell signals to promote myogenesis.	bind
25275	5	7883	6	NULL	NULL	0	NULL	statement 3	NULL		occurs via	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_5_1535_s_115	12414501	35  IGF-BP3 binds the IGFs and prevents the activation of the IGF-1 receptor, which normally mediates cell signals to promote myogenesis.	bind
32813	1	7884	5	13	NULL	NULL	NULL	MEKK1	GP	dominant-interfering	inhibits					ERK	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_167_s_220	9686756	35  In order to establish that inhibition of ERK activation by dominant-interfering MEKK1 is not responsible for the inhibitory effect on genetic markers of hypertrophic growth, we performed parallel experiments using dominant-interfering Raf-1, which binds Ras and inhibits the MEK/ERK pathway.	bind
32816	2	7884	5	13	NULL	NULL	NULL	Raf-1	GP	dominant-interfering	bind					Ras	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_167_s_220	9686756	35  In order to establish that inhibition of ERK activation by dominant-interfering MEKK1 is not responsible for the inhibitory effect on genetic markers of hypertrophic growth, we performed parallel experiments using dominant-interfering Raf-1, which binds Ras and inhibits the MEK/ERK pathway.	bind
32817	3	7884	5	13	NULL	NULL	NULL	statement 2	Process		inhibits					MEK/ERK pathway	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_2_167_s_220	9686756	35  In order to establish that inhibition of ERK activation by dominant-interfering MEKK1 is not responsible for the inhibitory effect on genetic markers of hypertrophic growth, we performed parallel experiments using dominant-interfering Raf-1, which binds Ras and inhibits the MEK/ERK pathway.	bind
25844	1	7884	6	NULL	NULL	0	NULL	MEKK1	NULL	dominant-interfering	inhibits	NULL				ERK	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_circulationres_83_2_167_s_220	9686756	35  In order to establish that inhibition of ERK activation by dominant-interfering MEKK1 is not responsible for the inhibitory effect on genetic markers of hypertrophic growth, we performed parallel experiments using dominant-interfering Raf-1, which binds Ras and inhibits the MEK/ERK pathway.	bind
25845	2	7884	6	NULL	NULL	0	NULL	Raf-1	NULL	dominant-interfering	bind	NULL				Ras	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_2_167_s_220	9686756	35  In order to establish that inhibition of ERK activation by dominant-interfering MEKK1 is not responsible for the inhibitory effect on genetic markers of hypertrophic growth, we performed parallel experiments using dominant-interfering Raf-1, which binds Ras and inhibits the MEK/ERK pathway.	bind
25846	3	7884	6	NULL	NULL	0	NULL	statement 2	NULL		inhibits	NULL				MEK/ERK pathway	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_2_167_s_220	9686756	35  In order to establish that inhibition of ERK activation by dominant-interfering MEKK1 is not responsible for the inhibitory effect on genetic markers of hypertrophic growth, we performed parallel experiments using dominant-interfering Raf-1, which binds Ras and inhibits the MEK/ERK pathway.	bind
32819	1	7885	5	13	NULL	NULL	NULL	TNF-alpha	GP		bind					ECM	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_14	12000736	35  On this basis, it is likely that TNF-alpha bound to ECM during processes of retinal fibrosis and neovascularization may affect Muller cell function, and hence influence the development of retinal proliferative disease.	bind
32820	2	7885	5	13	NULL	NULL	NULL	statement 1	Process		occurs during					retinal fibrosis	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_14	12000736	35  On this basis, it is likely that TNF-alpha bound to ECM during processes of retinal fibrosis and neovascularization may affect Muller cell function, and hence influence the development of retinal proliferative disease.	bind
32821	3	7885	5	13	NULL	NULL	NULL	statement 1	Process		occurs during					neovascularization	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_14	12000736	35  On this basis, it is likely that TNF-alpha bound to ECM during processes of retinal fibrosis and neovascularization may affect Muller cell function, and hence influence the development of retinal proliferative disease.	bind
32823	4	7885	5	13	NULL	NULL	NULL	statement 2	Process		affects		may			Muller cell 	Cell	function of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_14	12000736	35  On this basis, it is likely that TNF-alpha bound to ECM during processes of retinal fibrosis and neovascularization may affect Muller cell function, and hence influence the development of retinal proliferative disease.	bind
32825	5	7885	5	13	NULL	NULL	NULL	statement 3	Process		affects		may			Muller cell	Cell	function of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_14	12000736	35  On this basis, it is likely that TNF-alpha bound to ECM during processes of retinal fibrosis and neovascularization may affect Muller cell function, and hence influence the development of retinal proliferative disease.	bind
32826	6	7885	5	13	NULL	NULL	NULL	statement 4	Process		influence					retinal proliferative disease	MedicalFinding	development of 			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_14	12000736	35  On this basis, it is likely that TNF-alpha bound to ECM during processes of retinal fibrosis and neovascularization may affect Muller cell function, and hence influence the development of retinal proliferative disease.	bind
32827	7	7885	5	13	NULL	NULL	NULL	statement 5	Process		influence					retinal proliferative disease	MedicalFinding	development of 			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_14	12000736	35  On this basis, it is likely that TNF-alpha bound to ECM during processes of retinal fibrosis and neovascularization may affect Muller cell function, and hence influence the development of retinal proliferative disease.	bind
25276	1	7885	6	NULL	NULL	0	NULL	TNF-alpha	NULL		bind	NULL				ECM	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_14	12000736	35  On this basis, it is likely that TNF-alpha bound to ECM during processes of retinal fibrosis and neovascularization may affect Muller cell function, and hence influence the development of retinal proliferative disease.	bind
25277	2	7885	6	NULL	NULL	0	NULL	statement 1	NULL		occurs during	NULL				retinal fibrosis	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_14	12000736	35  On this basis, it is likely that TNF-alpha bound to ECM during processes of retinal fibrosis and neovascularization may affect Muller cell function, and hence influence the development of retinal proliferative disease.	bind
25278	3	7885	6	NULL	NULL	0	NULL	statement 1	NULL		occurs during	NULL				neovascularization	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_14	12000736	35  On this basis, it is likely that TNF-alpha bound to ECM during processes of retinal fibrosis and neovascularization may affect Muller cell function, and hence influence the development of retinal proliferative disease.	bind
25279	4	7885	6	10	NULL	0	NULL	statement 2			affect		may			Muller cell		function of 			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_14	12000736	35  On this basis, it is likely that TNF-alpha bound to ECM during processes of retinal fibrosis and neovascularization may affect Muller cell function, and hence influence the development of retinal proliferative disease.	bind
25280	5	7885	6	10	NULL	0	NULL	statement 3			affects		may			Muller cell		function of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_14	12000736	35  On this basis, it is likely that TNF-alpha bound to ECM during processes of retinal fibrosis and neovascularization may affect Muller cell function, and hence influence the development of retinal proliferative disease.	bind
55573	6	7885	6	10	NULL	0	NULL	statement 4			influences					retinal proliferative disease		development of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_14	12000736	35  On this basis, it is likely that TNF-alpha bound to ECM during processes of retinal fibrosis and neovascularization may affect Muller cell function, and hence influence the development of retinal proliferative disease.	bind
55574	7	7885	6	10	NULL	0	NULL	statement 5			influences					retinal proliferative disease		development of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_5_1847_s_14	12000736	35  On this basis, it is likely that TNF-alpha bound to ECM during processes of retinal fibrosis and neovascularization may affect Muller cell function, and hence influence the development of retinal proliferative disease.	bind
32828	1	7886	5	13	NULL	NULL	NULL	platelet glycoprotein IIb/IIa complex	GP		bind					fibrinogen	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3461_s_203	9437193	35 36  Platelet glycoprotein IIb/IIa complex provides binding sites for fibrinogen, 37 38  Fn, 39  vWF, 40  and also for Vn. 41  All these ligands react with platelet glycoprotein IIb/IIa complex only after platelet activation in a divalent cation - dependent manner, and the binding is inhibited by peptides containing an Arg-Gly-Asp sequence.	bind
32829	2	7886	5	13	NULL	NULL	NULL	platelet glycoprotein IIb/IIa complex	GP		bind					Fn	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3461_s_203	9437193	35 36  Platelet glycoprotein IIb/IIa complex provides binding sites for fibrinogen, 37 38  Fn, 39  vWF, 40  and also for Vn. 41  All these ligands react with platelet glycoprotein IIb/IIa complex only after platelet activation in a divalent cation - dependent manner, and the binding is inhibited by peptides containing an Arg-Gly-Asp sequence.	bind
32830	3	7886	5	13	NULL	NULL	NULL	platelet glycoprotein IIb/IIa complex	GP		bind					vWF	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3461_s_203	9437193	35 36  Platelet glycoprotein IIb/IIa complex provides binding sites for fibrinogen, 37 38  Fn, 39  vWF, 40  and also for Vn. 41  All these ligands react with platelet glycoprotein IIb/IIa complex only after platelet activation in a divalent cation - dependent manner, and the binding is inhibited by peptides containing an Arg-Gly-Asp sequence.	bind
32831	4	7886	5	13	NULL	NULL	NULL	platelet glycoprotein IIb/IIa complex	GP		bind					Vn	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3461_s_203	9437193	35 36  Platelet glycoprotein IIb/IIa complex provides binding sites for fibrinogen, 37 38  Fn, 39  vWF, 40  and also for Vn. 41  All these ligands react with platelet glycoprotein IIb/IIa complex only after platelet activation in a divalent cation - dependent manner, and the binding is inhibited by peptides containing an Arg-Gly-Asp sequence.	bind
32832	5	7886	5	13	NULL	NULL	NULL	platelet	Cell	activation of	is dependent on					divalent cation	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3461_s_203	9437193	35 36  Platelet glycoprotein IIb/IIa complex provides binding sites for fibrinogen, 37 38  Fn, 39  vWF, 40  and also for Vn. 41  All these ligands react with platelet glycoprotein IIb/IIa complex only after platelet activation in a divalent cation - dependent manner, and the binding is inhibited by peptides containing an Arg-Gly-Asp sequence.	bind
32833	6	7886	5	13	NULL	NULL	NULL	statement 5	Process		is required for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3461_s_203	9437193	35 36  Platelet glycoprotein IIb/IIa complex provides binding sites for fibrinogen, 37 38  Fn, 39  vWF, 40  and also for Vn. 41  All these ligands react with platelet glycoprotein IIb/IIa complex only after platelet activation in a divalent cation - dependent manner, and the binding is inhibited by peptides containing an Arg-Gly-Asp sequence.	bind
32834	7	7886	5	13	NULL	NULL	NULL	statement 5	Process		is required for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3461_s_203	9437193	35 36  Platelet glycoprotein IIb/IIa complex provides binding sites for fibrinogen, 37 38  Fn, 39  vWF, 40  and also for Vn. 41  All these ligands react with platelet glycoprotein IIb/IIa complex only after platelet activation in a divalent cation - dependent manner, and the binding is inhibited by peptides containing an Arg-Gly-Asp sequence.	bind
32835	8	7886	5	13	NULL	NULL	NULL	statement 5	Process		is required for					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3461_s_203	9437193	35 36  Platelet glycoprotein IIb/IIa complex provides binding sites for fibrinogen, 37 38  Fn, 39  vWF, 40  and also for Vn. 41  All these ligands react with platelet glycoprotein IIb/IIa complex only after platelet activation in a divalent cation - dependent manner, and the binding is inhibited by peptides containing an Arg-Gly-Asp sequence.	bind
32836	9	7886	5	13	NULL	NULL	NULL	statement 5	Process		is required for					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3461_s_203	9437193	35 36  Platelet glycoprotein IIb/IIa complex provides binding sites for fibrinogen, 37 38  Fn, 39  vWF, 40  and also for Vn. 41  All these ligands react with platelet glycoprotein IIb/IIa complex only after platelet activation in a divalent cation - dependent manner, and the binding is inhibited by peptides containing an Arg-Gly-Asp sequence.	bind
32837	10	7886	5	13	NULL	NULL	NULL	peptides	GP		inhibits			containing Arg-Gly-Asp sequence		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3461_s_203	9437193	35 36  Platelet glycoprotein IIb/IIa complex provides binding sites for fibrinogen, 37 38  Fn, 39  vWF, 40  and also for Vn. 41  All these ligands react with platelet glycoprotein IIb/IIa complex only after platelet activation in a divalent cation - dependent manner, and the binding is inhibited by peptides containing an Arg-Gly-Asp sequence.	bind
32838	11	7886	5	13	NULL	NULL	NULL	peptides	GP		inhibits			containing Arg-Gly-Asp sequence		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3461_s_203	9437193	35 36  Platelet glycoprotein IIb/IIa complex provides binding sites for fibrinogen, 37 38  Fn, 39  vWF, 40  and also for Vn. 41  All these ligands react with platelet glycoprotein IIb/IIa complex only after platelet activation in a divalent cation - dependent manner, and the binding is inhibited by peptides containing an Arg-Gly-Asp sequence.	bind
32839	12	7886	5	13	NULL	NULL	NULL	peptides	GP		inhibits			containing Arg-Gly-Asp sequence		statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3461_s_203	9437193	35 36  Platelet glycoprotein IIb/IIa complex provides binding sites for fibrinogen, 37 38  Fn, 39  vWF, 40  and also for Vn. 41  All these ligands react with platelet glycoprotein IIb/IIa complex only after platelet activation in a divalent cation - dependent manner, and the binding is inhibited by peptides containing an Arg-Gly-Asp sequence.	bind
32840	13	7886	5	13	NULL	NULL	NULL	peptides	GP		inhibits			containing Arg-Gly-Asp sequence		statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3461_s_203	9437193	35 36  Platelet glycoprotein IIb/IIa complex provides binding sites for fibrinogen, 37 38  Fn, 39  vWF, 40  and also for Vn. 41  All these ligands react with platelet glycoprotein IIb/IIa complex only after platelet activation in a divalent cation - dependent manner, and the binding is inhibited by peptides containing an Arg-Gly-Asp sequence.	bind
25747	1	7886	6	NULL	NULL	0	NULL	fibrinogen	NULL		react with	NULL				platelet glycoprotein IIb/IIa complex	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3461_s_203	9437193	35 36  Platelet glycoprotein IIb/IIa complex provides binding sites for fibrinogen, 37 38  Fn, 39  vWF, 40  and also for Vn. 41  All these ligands react with platelet glycoprotein IIb/IIa complex only after platelet activation in a divalent cation - dependent manner, and the binding is inhibited by peptides containing an Arg-Gly-Asp sequence.	bind
25748	2	7886	6	NULL	NULL	0	NULL	Fn	NULL		react with	NULL				platelet glycoprotein IIb/IIa complex	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3461_s_203	9437193	35 36  Platelet glycoprotein IIb/IIa complex provides binding sites for fibrinogen, 37 38  Fn, 39  vWF, 40  and also for Vn. 41  All these ligands react with platelet glycoprotein IIb/IIa complex only after platelet activation in a divalent cation - dependent manner, and the binding is inhibited by peptides containing an Arg-Gly-Asp sequence.	bind
25749	3	7886	6	NULL	NULL	0	NULL	vWF	NULL		react with	NULL				platelet glycoprotein IIb/IIa complex	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3461_s_203	9437193	35 36  Platelet glycoprotein IIb/IIa complex provides binding sites for fibrinogen, 37 38  Fn, 39  vWF, 40  and also for Vn. 41  All these ligands react with platelet glycoprotein IIb/IIa complex only after platelet activation in a divalent cation - dependent manner, and the binding is inhibited by peptides containing an Arg-Gly-Asp sequence.	bind
25751	4	7886	6	NULL	NULL	0	NULL	Vn	NULL		react with	NULL				platelet glycoprotein IIb/IIa complex	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3461_s_203	9437193	35 36  Platelet glycoprotein IIb/IIa complex provides binding sites for fibrinogen, 37 38  Fn, 39  vWF, 40  and also for Vn. 41  All these ligands react with platelet glycoprotein IIb/IIa complex only after platelet activation in a divalent cation - dependent manner, and the binding is inhibited by peptides containing an Arg-Gly-Asp sequence.	bind
25835	5	7886	6	NULL	NULL	0	NULL	statement 1	NULL		occurs after	NULL	only			platelet	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3461_s_203	9437193	35 36  Platelet glycoprotein IIb/IIa complex provides binding sites for fibrinogen, 37 38  Fn, 39  vWF, 40  and also for Vn. 41  All these ligands react with platelet glycoprotein IIb/IIa complex only after platelet activation in a divalent cation - dependent manner, and the binding is inhibited by peptides containing an Arg-Gly-Asp sequence.	bind
25836	6	7886	6	NULL	NULL	0	NULL	platelet	NULL	activation of	is dependent on	NULL				divalent cation	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3461_s_203	9437193	35 36  Platelet glycoprotein IIb/IIa complex provides binding sites for fibrinogen, 37 38  Fn, 39  vWF, 40  and also for Vn. 41  All these ligands react with platelet glycoprotein IIb/IIa complex only after platelet activation in a divalent cation - dependent manner, and the binding is inhibited by peptides containing an Arg-Gly-Asp sequence.	bind
25837	7	7886	6	NULL	NULL	0	NULL	statement 2	NULL		occurs after	NULL	only			platelet	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3461_s_203	9437193	35 36  Platelet glycoprotein IIb/IIa complex provides binding sites for fibrinogen, 37 38  Fn, 39  vWF, 40  and also for Vn. 41  All these ligands react with platelet glycoprotein IIb/IIa complex only after platelet activation in a divalent cation - dependent manner, and the binding is inhibited by peptides containing an Arg-Gly-Asp sequence.	bind
25838	8	7886	6	NULL	NULL	0	NULL	statement 3	NULL		occurs after	NULL	only			platelets	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3461_s_203	9437193	35 36  Platelet glycoprotein IIb/IIa complex provides binding sites for fibrinogen, 37 38  Fn, 39  vWF, 40  and also for Vn. 41  All these ligands react with platelet glycoprotein IIb/IIa complex only after platelet activation in a divalent cation - dependent manner, and the binding is inhibited by peptides containing an Arg-Gly-Asp sequence.	bind
25839	9	7886	6	NULL	NULL	0	NULL	statement 4	NULL		occurs after	NULL	only			platelets	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3461_s_203	9437193	35 36  Platelet glycoprotein IIb/IIa complex provides binding sites for fibrinogen, 37 38  Fn, 39  vWF, 40  and also for Vn. 41  All these ligands react with platelet glycoprotein IIb/IIa complex only after platelet activation in a divalent cation - dependent manner, and the binding is inhibited by peptides containing an Arg-Gly-Asp sequence.	bind
25840	10	7886	6	NULL	NULL	0	NULL	statement 1	NULL		is inhibited by	NULL				peptides	NULL		Arg-Gly-Asp sequence		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3461_s_203	9437193	35 36  Platelet glycoprotein IIb/IIa complex provides binding sites for fibrinogen, 37 38  Fn, 39  vWF, 40  and also for Vn. 41  All these ligands react with platelet glycoprotein IIb/IIa complex only after platelet activation in a divalent cation - dependent manner, and the binding is inhibited by peptides containing an Arg-Gly-Asp sequence.	bind
25841	11	7886	6	NULL	NULL	0	NULL	statement 2	NULL		is inhibited by	NULL				peptides	NULL		Arg-Gly-Asp sequence		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3461_s_203	9437193	35 36  Platelet glycoprotein IIb/IIa complex provides binding sites for fibrinogen, 37 38  Fn, 39  vWF, 40  and also for Vn. 41  All these ligands react with platelet glycoprotein IIb/IIa complex only after platelet activation in a divalent cation - dependent manner, and the binding is inhibited by peptides containing an Arg-Gly-Asp sequence.	bind
25842	12	7886	6	NULL	NULL	0	NULL	statement 3	NULL		is inhibited by	NULL				peptides	NULL		Arg-Gly-Asp sequence		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3461_s_203	9437193	35 36  Platelet glycoprotein IIb/IIa complex provides binding sites for fibrinogen, 37 38  Fn, 39  vWF, 40  and also for Vn. 41  All these ligands react with platelet glycoprotein IIb/IIa complex only after platelet activation in a divalent cation - dependent manner, and the binding is inhibited by peptides containing an Arg-Gly-Asp sequence.	bind
25843	13	7886	6	NULL	NULL	0	NULL	statement 4	NULL		is inhibited by	NULL				peptides	NULL		Arg-Gly-Asp sequence		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3461_s_203	9437193	35 36  Platelet glycoprotein IIb/IIa complex provides binding sites for fibrinogen, 37 38  Fn, 39  vWF, 40  and also for Vn. 41  All these ligands react with platelet glycoprotein IIb/IIa complex only after platelet activation in a divalent cation - dependent manner, and the binding is inhibited by peptides containing an Arg-Gly-Asp sequence.	bind
32841	1	7887	5	13	NULL	NULL	NULL	CD40L	GP		bind					CD40 	GP				NULL	on endothelium	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1321_s_100	15831808	35 CD40L binding to CD40 on endothelium induces inflammation, and this biological activity is also preserved in platelet CD40L.	bind
32842	2	7887	5	13	NULL	NULL	NULL	statement 1	Process		induces					inflammation	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1321_s_100	15831808	35 CD40L binding to CD40 on endothelium induces inflammation, and this biological activity is also preserved in platelet CD40L.	bind
32843	3	7887	5	13	NULL	NULL	NULL	CD40L	GP	platelet 	bind					CD40	GP				NULL	on endothelium	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1321_s_100	15831808	35 CD40L binding to CD40 on endothelium induces inflammation, and this biological activity is also preserved in platelet CD40L.	bind
32844	4	7887	5	13	NULL	NULL	NULL	statement 3	Process		induces					inflammation	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1321_s_100	15831808	35 CD40L binding to CD40 on endothelium induces inflammation, and this biological activity is also preserved in platelet CD40L.	bind
25281	1	7887	6	NULL	NULL	0	NULL	CD40L	NULL		bind	NULL				CD40	NULL				NULL	endothelium	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1321_s_100	15831808	35 CD40L binding to CD40 on endothelium induces inflammation, and this biological activity is also preserved in platelet CD40L.	bind
25282	2	7887	6	NULL	NULL	0	NULL	statement 1	NULL		induces	NULL				inflammation	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1321_s_100	15831808	35 CD40L binding to CD40 on endothelium induces inflammation, and this biological activity is also preserved in platelet CD40L.	bind
25283	3	7887	6	NULL	NULL	0	NULL	CD40L	NULL	platelet	bind	NULL				CD40	NULL				NULL	endothelium	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1321_s_100	15831808	35 CD40L binding to CD40 on endothelium induces inflammation, and this biological activity is also preserved in platelet CD40L.	bind
25284	4	7887	6	NULL	NULL	0	NULL	statement 3	NULL		induces	NULL				inflammation	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1321_s_100	15831808	35 CD40L binding to CD40 on endothelium induces inflammation, and this biological activity is also preserved in platelet CD40L.	bind
32846	1	7888	5	13	NULL	NULL	NULL	p300	GP		bind					p160 member	GP		AD1 domain		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_703_s_166	14764426	35 Concomitantly, p300 (or CBP) binds to the AD1 domain of the p160 member.	bind
32848	2	7888	5	13	NULL	NULL	NULL	CBP	GP		bind					p160 member	GP		AD1 domain		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_703_s_166	14764426	35 Concomitantly, p300 (or CBP) binds to the AD1 domain of the p160 member.	bind
32849	3	7888	5	13	NULL	NULL	NULL	statement 1	Process		is alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_703_s_166	14764426	35 Concomitantly, p300 (or CBP) binds to the AD1 domain of the p160 member.	bind
25285	1	7888	6	NULL	NULL	0	NULL	p300	NULL		bind	NULL	concomitantly			p160	NULL		AD1 domain		NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_703_s_166	14764426	35 Concomitantly, p300 (or CBP) binds to the AD1 domain of the p160 member.	bind
25286	2	7888	6	NULL	NULL	0	NULL	CBP	NULL		bind	NULL	concomitantly			p160	NULL		AD1 domain		NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_703_s_166	14764426	35 Concomitantly, p300 (or CBP) binds to the AD1 domain of the p160 member.	bind
47549	3	7888	6	10	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_4_703_s_166	14764426	35 Concomitantly, p300 (or CBP) binds to the AD1 domain of the p160 member.	bind
32851	1	7889	5	13	NULL	NULL	NULL	serum response factor	GP		bind									CArG element	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_2_158_s_207	11834708	35 Gel-mobility supershift analysis demonstrated that the serum response factor binds to the CArG element and that GATA-4 binds to the GATA element.	bind
32852	2	7889	5	13	NULL	NULL	NULL	GATA-4	GP		bind									GATA element	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_2_158_s_207	11834708	35 Gel-mobility supershift analysis demonstrated that the serum response factor binds to the CArG element and that GATA-4 binds to the GATA element.	bind
25287	1	7889	6	NULL	NULL	0	NULL	serum response factor	NULL		bind	NULL					NULL			CArG element	NULL		0	NULL	NULL	NULL	gw60_circulationres_90_2_158_s_207	11834708	35 Gel-mobility supershift analysis demonstrated that the serum response factor binds to the CArG element and that GATA-4 binds to the GATA element.	bind
25288	2	7889	6	NULL	NULL	0	NULL	GATA-4	NULL		bind	NULL					NULL			GATA element	NULL		0	NULL	NULL	NULL	gw60_circulationres_90_2_158_s_207	11834708	35 Gel-mobility supershift analysis demonstrated that the serum response factor binds to the CArG element and that GATA-4 binds to the GATA element.	bind
32854	1	7890	5	13	NULL	NULL	NULL	TNF-alpha	GP		induces					AP-1	GP	binding activity of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_334_s_183	15576639	35 In this study, SOD overexpression suppressed the increase in AP-1 and NF-kappaB binding activity induced by TNF-alpha.	bind
32855	2	7890	5	13	NULL	NULL	NULL	TNF-alpha	GP		induces					NF-kappaB	GP	binding activity of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_334_s_183	15576639	35 In this study, SOD overexpression suppressed the increase in AP-1 and NF-kappaB binding activity induced by TNF-alpha.	bind
32857	3	7890	5	13	NULL	NULL	NULL	SOD	GP	overexpression of	supress					statement 1	Process	increase in			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_334_s_183	15576639	35 In this study, SOD overexpression suppressed the increase in AP-1 and NF-kappaB binding activity induced by TNF-alpha.	bind
32858	4	7890	5	13	NULL	NULL	NULL	SOD	GP	overexpression of	supress					statement 2	Process	increase in			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_334_s_183	15576639	35 In this study, SOD overexpression suppressed the increase in AP-1 and NF-kappaB binding activity induced by TNF-alpha.	bind
25289	1	7890	6	NULL	NULL	0	NULL	TNF-alpha	NULL		induce	NULL				AP-1	NULL	binding activity of 			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_334_s_183	15576639	35 In this study, SOD overexpression suppressed the increase in AP-1 and NF-kappaB binding activity induced by TNF-alpha.	bind
25290	2	7890	6	NULL	NULL	0	NULL	TNF-alpha	NULL		induce	NULL				NF-kappaB	NULL	binding activity of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_334_s_183	15576639	35 In this study, SOD overexpression suppressed the increase in AP-1 and NF-kappaB binding activity induced by TNF-alpha.	bind
25291	3	7890	6	NULL	NULL	0	NULL	SOD	NULL	overexpression of	suppresses	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_334_s_183	15576639	35 In this study, SOD overexpression suppressed the increase in AP-1 and NF-kappaB binding activity induced by TNF-alpha.	bind
38870	4	7890	6	NULL	NULL	0	NULL	SOD	NULL	overexpression of	suppresses	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_2_334_s_183	15576639	35 In this study, SOD overexpression suppressed the increase in AP-1 and NF-kappaB binding activity induced by TNF-alpha.	bind
32870	2	7891	5	13	NULL	NULL	NULL	statement 1	GP		bind					target genes	GP			XRE	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1652_s_206	15271786	35 It is a ligand-activated transcription factor that binds to the XRE of target genes regulating expression of a number of xenobiotic-metabolizing enzymes.	bind
32871	3	7891	5	13	NULL	NULL	NULL	statement 2	Process		regulates					xenobiotic-metabolizing enzymes	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1652_s_206	15271786	35 It is a ligand-activated transcription factor that binds to the XRE of target genes regulating expression of a number of xenobiotic-metabolizing enzymes.	bind
47550	1	7891	5	13	NULL	NULL	NULL	ligand	GP		activates					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1652_s_206	15271786	35 It is a ligand-activated transcription factor that binds to the XRE of target genes regulating expression of a number of xenobiotic-metabolizing enzymes.	bind
25292	2	7891	6	10	NULL	0	NULL	statement 1	NULL		bind	NULL				target genes	NULL			XRE	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1652_s_206	15271786	35 It is a ligand-activated transcription factor that binds to the XRE of target genes regulating expression of a number of xenobiotic-metabolizing enzymes.	bind
25293	3	7891	6	10	NULL	0	NULL	statement 2	NULL		regulate	NULL				xenobiotic-metabolizing enzymes	NULL	expression of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1652_s_206	15271786	35 It is a ligand-activated transcription factor that binds to the XRE of target genes regulating expression of a number of xenobiotic-metabolizing enzymes.	bind
47551	1	7891	6	10	NULL	0	NULL	ligand	NULL		activates	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1652_s_206	15271786	35 It is a ligand-activated transcription factor that binds to the XRE of target genes regulating expression of a number of xenobiotic-metabolizing enzymes.	bind
32872	1	7893	5	13	NULL	NULL	NULL	Pex5p	GP	35 S-Labeled	bind		dose dependent			Pex13p	GP		SH3 domain		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_6_4127_s_146	10660573	35 S-Labeled Pex5p binding to the Pex13p  SH3  domain  in vitro occurs in a dose-dependent manner and is inhibited by the addition of unlabeled Pex5p.	bind
32873	2	7893	5	13	NULL	NULL	NULL	Pex5p	GP	unlabeled	inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_6_4127_s_146	10660573	35 S-Labeled Pex5p binding to the Pex13p  SH3  domain  in vitro occurs in a dose-dependent manner and is inhibited by the addition of unlabeled Pex5p.	bind
25294	1	7893	6	NULL	NULL	0	NULL	Pex5p	NULL	35 S-labeled	bind	NULL	dose dependently			Pex13p	NULL		SH3 domain		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_6_4127_s_146	10660573	35 S-Labeled Pex5p binding to the Pex13p  SH3  domain  in vitro occurs in a dose-dependent manner and is inhibited by the addition of unlabeled Pex5p.	bind
25295	2	7893	6	NULL	NULL	0	NULL	Pex5p	NULL	unlabeled	inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_6_4127_s_146	10660573	35 S-Labeled Pex5p binding to the Pex13p  SH3  domain  in vitro occurs in a dose-dependent manner and is inhibited by the addition of unlabeled Pex5p.	bind
32874	1	7895	5	13	NULL	NULL	NULL	AML1	GP	35S-labeled	bind					GST-MEF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3635_s_104	10207087	35S-labeled AML1, AML1B, AML1/ETO, and TEL/AML1 [the oncogenic product generated by the t(12;21) translocation in childhood acute lymphoblastic leukemia] bound to GST-MEF (lanes 2, 4, 6, and 8) but not to GST alone (lanes 1, 3, 5, and 7).	bind
32876	2	7895	5	13	NULL	NULL	NULL	AML1B	GP	35S-labeled	bind					GST-MEF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3635_s_104	10207087	35S-labeled AML1, AML1B, AML1/ETO, and TEL/AML1 [the oncogenic product generated by the t(12;21) translocation in childhood acute lymphoblastic leukemia] bound to GST-MEF (lanes 2, 4, 6, and 8) but not to GST alone (lanes 1, 3, 5, and 7).	bind
32878	3	7895	5	13	NULL	NULL	NULL	AML1/ETO	GP	35S-labeled	bind					GST-MEF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3635_s_104	10207087	35S-labeled AML1, AML1B, AML1/ETO, and TEL/AML1 [the oncogenic product generated by the t(12;21) translocation in childhood acute lymphoblastic leukemia] bound to GST-MEF (lanes 2, 4, 6, and 8) but not to GST alone (lanes 1, 3, 5, and 7).	bind
32880	4	7895	5	13	NULL	NULL	NULL	TEL/AML1	GP	35S-labeled	bind					GST-MEF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3635_s_104	10207087	35S-labeled AML1, AML1B, AML1/ETO, and TEL/AML1 [the oncogenic product generated by the t(12;21) translocation in childhood acute lymphoblastic leukemia] bound to GST-MEF (lanes 2, 4, 6, and 8) but not to GST alone (lanes 1, 3, 5, and 7).	bind
38973	5	7895	5	13	NULL	NULL	NULL	TEL/AML1	GP		is a type of					oncogenic product	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3635_s_104	10207087	35S-labeled AML1, AML1B, AML1/ETO, and TEL/AML1 [the oncogenic product generated by the t(12;21) translocation in childhood acute lymphoblastic leukemia] bound to GST-MEF (lanes 2, 4, 6, and 8) but not to GST alone (lanes 1, 3, 5, and 7).	bind
25296	1	7895	6	NULL	NULL	0	NULL	AML1	NULL	35S-labeled	bind	NULL				GST-MEF	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3635_s_104	10207087	35S-labeled AML1, AML1B, AML1/ETO, and TEL/AML1 [the oncogenic product generated by the t(12;21) translocation in childhood acute lymphoblastic leukemia] bound to GST-MEF (lanes 2, 4, 6, and 8) but not to GST alone (lanes 1, 3, 5, and 7).	bind
25297	2	7895	6	NULL	NULL	0	NULL	AML1B	NULL	35S-labeled	bind	NULL				GST-MEF	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3635_s_104	10207087	35S-labeled AML1, AML1B, AML1/ETO, and TEL/AML1 [the oncogenic product generated by the t(12;21) translocation in childhood acute lymphoblastic leukemia] bound to GST-MEF (lanes 2, 4, 6, and 8) but not to GST alone (lanes 1, 3, 5, and 7).	bind
25298	3	7895	6	NULL	NULL	0	NULL	AML1/ETO	NULL	35S-labeled	bind	NULL				GST-MEF	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3635_s_104	10207087	35S-labeled AML1, AML1B, AML1/ETO, and TEL/AML1 [the oncogenic product generated by the t(12;21) translocation in childhood acute lymphoblastic leukemia] bound to GST-MEF (lanes 2, 4, 6, and 8) but not to GST alone (lanes 1, 3, 5, and 7).	bind
25299	4	7895	6	NULL	NULL	0	NULL	TEL/AML1	NULL	35S-labeled	bind	NULL				GST-MEF	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3635_s_104	10207087	35S-labeled AML1, AML1B, AML1/ETO, and TEL/AML1 [the oncogenic product generated by the t(12;21) translocation in childhood acute lymphoblastic leukemia] bound to GST-MEF (lanes 2, 4, 6, and 8) but not to GST alone (lanes 1, 3, 5, and 7).	bind
25746	5	7895	6	NULL	NULL	0	NULL	TEL/AML1	NULL		is a type of	NULL				oncogenic product	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3635_s_104	10207087	35S-labeled AML1, AML1B, AML1/ETO, and TEL/AML1 [the oncogenic product generated by the t(12;21) translocation in childhood acute lymphoblastic leukemia] bound to GST-MEF (lanes 2, 4, 6, and 8) but not to GST alone (lanes 1, 3, 5, and 7).	bind
32882	1	7896	5	13	NULL	NULL	NULL	AP1	GP	35S-labeled	bind					SEU-GST	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_133_16_3159_s_116	16854969	35S-labeled AP1, SEP3 or AP3 was bound to SEU-GST resins.	bind
32883	2	7896	5	13	NULL	NULL	NULL	SEP3	GP	35S-labeled	bind					SEU-GST	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_133_16_3159_s_116	16854969	35S-labeled AP1, SEP3 or AP3 was bound to SEU-GST resins.	bind
32884	3	7896	5	13	NULL	NULL	NULL	AP3	GP	35S-labeled	bind					SEU-GST	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_133_16_3159_s_116	16854969	35S-labeled AP1, SEP3 or AP3 was bound to SEU-GST resins.	bind
25300	1	7896	6	NULL	NULL	0	NULL	AP1	NULL	35S-labeled	bind	NULL				SEU-GST resin	NULL				NULL		0	NULL	NULL	NULL	gw70_development_133_16_3159_s_116	16854969	35S-labeled AP1, SEP3 or AP3 was bound to SEU-GST resins.	bind
25301	2	7896	6	NULL	NULL	0	NULL	SEP3	NULL	35S-labeled	bind	NULL				SEU-GST resin	NULL				NULL		0	NULL	NULL	NULL	gw70_development_133_16_3159_s_116	16854969	35S-labeled AP1, SEP3 or AP3 was bound to SEU-GST resins.	bind
25302	3	7896	6	NULL	NULL	0	NULL	AP3	NULL	35S-labeled	bind	NULL				SEU-GST resin	NULL				NULL		0	NULL	NULL	NULL	gw70_development_133_16_3159_s_116	16854969	35S-labeled AP1, SEP3 or AP3 was bound to SEU-GST resins.	bind
32885	1	7897	5	13	NULL	NULL	NULL	Arp1	GP	35S-labeled	bind					DI constructs	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_39_36598_s_99	11461920	35S-Labeled Arp1 bound to both the DI and DIII constructs but did not bind significantly to the DII construct or to the GST control column (Fig.  2 a).	bind
32886	2	7897	5	13	NULL	NULL	NULL	Arp1	GP	35S-labeled	bind					DIII constructs	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_39_36598_s_99	11461920	35S-Labeled Arp1 bound to both the DI and DIII constructs but did not bind significantly to the DII construct or to the GST control column (Fig.  2 a).	bind
32887	3	7897	5	13	NULL	NULL	NULL	Arp1	GP	35S-labeled	does not bind		significantly			DII construct	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_39_36598_s_99	11461920	35S-Labeled Arp1 bound to both the DI and DIII constructs but did not bind significantly to the DII construct or to the GST control column (Fig.  2 a).	bind
25303	1	7897	6	NULL	NULL	0	NULL	Arp1	NULL	35S-labeled	bind	NULL				DI construct	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_39_36598_s_99	11461920	35S-Labeled Arp1 bound to both the DI and DIII constructs but did not bind significantly to the DII construct or to the GST control column (Fig.  2 a).	bind
25304	2	7897	6	NULL	NULL	0	NULL	Arp1	NULL	35S-labeled	bind	NULL				DIII construct	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_39_36598_s_99	11461920	35S-Labeled Arp1 bound to both the DI and DIII constructs but did not bind significantly to the DII construct or to the GST control column (Fig.  2 a).	bind
25305	3	7897	6	NULL	NULL	0	NULL	Arp1	NULL	35S-labeled	did not bind	NULL	significantly			DII construct	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_39_36598_s_99	11461920	35S-Labeled Arp1 bound to both the DI and DIII constructs but did not bind significantly to the DII construct or to the GST control column (Fig.  2 a).	bind
32889	1	7898	5	13	NULL	NULL	NULL	Arr2	GP	35S-labeled	bind					PIP3	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neuron_39_1_121_s_108	12848937	35S-labeled Arr2 bound to PIP3 beads but not to control beads   (Figure 2D).	bind
25306	1	7898	6	NULL	NULL	0	NULL	Arr2	NULL	35S-labeled	bind	NULL				PIP3	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_39_1_121_s_108	12848937	35S-labeled Arr2 bound to PIP3 beads but not to control beads   (Figure 2D).	bind
32890	1	7899	5	13	NULL	NULL	NULL	BAX	GP	35S-labeled	bind					GST-BCL-xL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_20_12415_s_120	9575197	35S-labeled BAX bound to GST-BCL-xL was analyzed by SDS-PAGE.	bind
25307	1	7899	6	NULL	NULL	0	NULL	BAX	NULL	35S-labeled	bind	NULL				GST-BCL-xL	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_20_12415_s_120	9575197	35S-labeled BAX bound to GST-BCL-xL was analyzed by SDS-PAGE.	bind
32891	1	7900	5	13	NULL	NULL	NULL	Cbfa2	GP	35S-labeled	bind					GST-Cbfbeta	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_4197_s_258	9632804	35S-labeled Cbfa2 was bound by immobilized GST-Cbfbeta but not by GST alone (Fig.  7A, lanes 4 to 6).	bind
32892	2	7900	5	13	NULL	NULL	NULL	Cbfa2	GP	35S-labeled	does not bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_4197_s_258	9632804	35S-labeled Cbfa2 was bound by immobilized GST-Cbfbeta but not by GST alone (Fig.  7A, lanes 4 to 6).	bind
25308	1	7900	6	NULL	NULL	0	NULL	Cbfa2	NULL	35S-labeled	bind	NULL				GST-Cbfbeta	NULL	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_4197_s_258	9632804	35S-labeled Cbfa2 was bound by immobilized GST-Cbfbeta but not by GST alone (Fig.  7A, lanes 4 to 6).	bind
25309	2	7900	6	NULL	NULL	0	NULL	Cbfa2	NULL	35S-labeled	does not bind	NULL				GST	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_7_4197_s_258	9632804	35S-labeled Cbfa2 was bound by immobilized GST-Cbfbeta but not by GST alone (Fig.  7A, lanes 4 to 6).	bind
32893	1	7901	5	13	NULL	NULL	NULL	Cdc20p	GP	35S-labeled	bind					MBP-Hsl1p	GP		667-872		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_18_2381_s_162	11562348	35S-labeled Cdc20p bound to MBP-Hsl1p667-872 and MBP-Hsl1p667-872mkb, but not to MBP alone or to MBP-Hsl1p667-872mdb (Fig.  6, top, left panel, lanes 1-4).	bind
32894	2	7901	5	13	NULL	NULL	NULL	Cdc20p	GP	35S-labeled	bind					MBP-Hsl1p	GP		667-872mkb		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_18_2381_s_162	11562348	35S-labeled Cdc20p bound to MBP-Hsl1p667-872 and MBP-Hsl1p667-872mkb, but not to MBP alone or to MBP-Hsl1p667-872mdb (Fig.  6, top, left panel, lanes 1-4).	bind
32895	3	7901	5	13	NULL	NULL	NULL	Cdc20p	GP	35S-labeled	does not bind					MBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_18_2381_s_162	11562348	35S-labeled Cdc20p bound to MBP-Hsl1p667-872 and MBP-Hsl1p667-872mkb, but not to MBP alone or to MBP-Hsl1p667-872mdb (Fig.  6, top, left panel, lanes 1-4).	bind
32896	4	7901	5	13	NULL	NULL	NULL	Cdc20p	GP	35S-labeled	does not bind					MBP-Hsl1p	GP		667-872mdb		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_18_2381_s_162	11562348	35S-labeled Cdc20p bound to MBP-Hsl1p667-872 and MBP-Hsl1p667-872mkb, but not to MBP alone or to MBP-Hsl1p667-872mdb (Fig.  6, top, left panel, lanes 1-4).	bind
25310	1	7901	6	NULL	NULL	0	NULL	Cdc20p	NULL	35S-labeled	bind	NULL				MBP-Hsl1	NULL		p667-872		NULL		0	NULL	NULL	NULL	gw60_genesdev_15_18_2381_s_162	11562348	35S-labeled Cdc20p bound to MBP-Hsl1p667-872 and MBP-Hsl1p667-872mkb, but not to MBP alone or to MBP-Hsl1p667-872mdb (Fig.  6, top, left panel, lanes 1-4).	bind
25311	2	7901	6	NULL	NULL	0	NULL	Cdc20p	NULL	35S-labeled	bind	NULL				MBP-Hsl1	NULL		p667-872mkb		NULL		0	NULL	NULL	NULL	gw60_genesdev_15_18_2381_s_162	11562348	35S-labeled Cdc20p bound to MBP-Hsl1p667-872 and MBP-Hsl1p667-872mkb, but not to MBP alone or to MBP-Hsl1p667-872mdb (Fig.  6, top, left panel, lanes 1-4).	bind
25312	3	7901	6	NULL	NULL	0	NULL	Cdc20p	NULL	35S-labeled	does not bind	NULL				MBP-Hsl1	NULL		p667-872mdb		NULL		0	NULL	NULL	NULL	gw60_genesdev_15_18_2381_s_162	11562348	35S-labeled Cdc20p bound to MBP-Hsl1p667-872 and MBP-Hsl1p667-872mkb, but not to MBP alone or to MBP-Hsl1p667-872mdb (Fig.  6, top, left panel, lanes 1-4).	bind
25313	4	7901	6	NULL	NULL	0	NULL	Cdc20p	NULL	35S-labeled	does not bind	NULL				MBP alone	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_15_18_2381_s_162	11562348	35S-labeled Cdc20p bound to MBP-Hsl1p667-872 and MBP-Hsl1p667-872mkb, but not to MBP alone or to MBP-Hsl1p667-872mdb (Fig.  6, top, left panel, lanes 1-4).	bind
32898	1	7902	5	13	NULL	NULL	NULL	dTopors	GP	35S-labeled	bind					GST-Hairy	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_17_17126_s_132	14871887	35S-Labeled dTopors (20% input;  lane 1) did not bind GST ( lane 2), but did bind GST-Hairy ( lane 3).	bind
25315	1	7902	6	NULL	NULL	0	NULL	dTopors	NULL	35S-labeled	bind	NULL				GST-Hairy	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_17_17126_s_132	14871887	35S-Labeled dTopors (20% input;  lane 1) did not bind GST ( lane 2), but did bind GST-Hairy ( lane 3).	bind
32900	1	7903	5	13	NULL	NULL	NULL	E2F1	GP	35S-labeled	bind					GST-Phb	GP		CC		NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_312_2_459_s_97	14637159	35S-labeled E2F1 does not bind to GST beads but binds to GST-Phb-CC beads.	bind
25317	1	7903	6	10	NULL	0	NULL	E2F1		35S-labeled	bind					GST-Phb			CC		NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_312_2_459_s_97	14637159	35S-labeled E2F1 does not bind to GST beads but binds to GST-Phb-CC beads.	bind
32901	1	7904	5	13	NULL	NULL	NULL	EBNA3C	GP	35S-labeled	bind					GST-ProTalpha protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5722_s_202	10891508	35S-labeled EBNA3C bound to GST-ProTalpha protein in this experiment at levels approximately 20-fold over binding with GST beads alone as determined by arbitrary counts using the Molecular Dynamics software ImageQuant supplied with the PhosphorImager unit (Fig.  3B, compare lane 3 with lane 5).	bind
25745	1	7904	6	NULL	NULL	0	NULL	EBNA3C	NULL	35S-labeled	bind	NULL				GST-ProTalpha protein	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_15_5722_s_202	10891508	35S-labeled EBNA3C bound to GST-ProTalpha protein in this experiment at levels approximately 20-fold over binding with GST beads alone as determined by arbitrary counts using the Molecular Dynamics software ImageQuant supplied with the PhosphorImager unit (Fig.  3B, compare lane 3 with lane 5).	bind
32902	1	7905	5	13	NULL	NULL	NULL	GSK3beta	GP	35S-labeled	bind					MEKK1	GP		N1 amino acids 1-401		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_16_13995_s_129	12584189	35S-Labeled GSK3beta bound to MEKK1-N1 (amino acids 1-401 of MEKK1) and MEKK1-N2 (amino acids 402-821) but not to MEKK1-deltaNC (amino acids 822-1172) or deltaMEKK1 (amino acids 1173-1493) (Fig.  5 A).	bind
32903	2	7905	5	13	NULL	NULL	NULL	GSK3beta	GP	35S-labeled	bind					MEKK1	GP		N2 amino acids 402-821		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_16_13995_s_129	12584189	35S-Labeled GSK3beta bound to MEKK1-N1 (amino acids 1-401 of MEKK1) and MEKK1-N2 (amino acids 402-821) but not to MEKK1-deltaNC (amino acids 822-1172) or deltaMEKK1 (amino acids 1173-1493) (Fig.  5 A).	bind
32904	3	7905	5	13	NULL	NULL	NULL	GSK3beta	GP	35S-labeled	does not bind					MEKK1	GP		deltaNC amino acids 822-1172		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_16_13995_s_129	12584189	35S-Labeled GSK3beta bound to MEKK1-N1 (amino acids 1-401 of MEKK1) and MEKK1-N2 (amino acids 402-821) but not to MEKK1-deltaNC (amino acids 822-1172) or deltaMEKK1 (amino acids 1173-1493) (Fig.  5 A).	bind
32905	4	7905	5	13	NULL	NULL	NULL	GSK3beta	GP	35S-labeled	does not bind					deltaMEKK1	GP		amino acids 1173-1493		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_16_13995_s_129	12584189	35S-Labeled GSK3beta bound to MEKK1-N1 (amino acids 1-401 of MEKK1) and MEKK1-N2 (amino acids 402-821) but not to MEKK1-deltaNC (amino acids 822-1172) or deltaMEKK1 (amino acids 1173-1493) (Fig.  5 A).	bind
25318	1	7905	6	NULL	NULL	0	NULL	GSK3beta	NULL	35S-labeled	bind	NULL				MEKK1-N1	NULL		amino acids 1-401		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_16_13995_s_129	12584189	35S-Labeled GSK3beta bound to MEKK1-N1 (amino acids 1-401 of MEKK1) and MEKK1-N2 (amino acids 402-821) but not to MEKK1-deltaNC (amino acids 822-1172) or deltaMEKK1 (amino acids 1173-1493) (Fig.  5 A).	bind
25319	2	7905	6	NULL	NULL	0	NULL	GSK3beta	NULL	35S-labeled	bind	NULL				MEKK1-N2	NULL		amino acids 402-821		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_16_13995_s_129	12584189	35S-Labeled GSK3beta bound to MEKK1-N1 (amino acids 1-401 of MEKK1) and MEKK1-N2 (amino acids 402-821) but not to MEKK1-deltaNC (amino acids 822-1172) or deltaMEKK1 (amino acids 1173-1493) (Fig.  5 A).	bind
25320	3	7905	6	NULL	NULL	0	NULL	GSK3beta	NULL	35S-labeled	does not bind	NULL				MEKK1-deltaNC	NULL		amino acids 822-1172		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_16_13995_s_129	12584189	35S-Labeled GSK3beta bound to MEKK1-N1 (amino acids 1-401 of MEKK1) and MEKK1-N2 (amino acids 402-821) but not to MEKK1-deltaNC (amino acids 822-1172) or deltaMEKK1 (amino acids 1173-1493) (Fig.  5 A).	bind
25339	4	7905	6	NULL	NULL	0	NULL	GSK3beta	NULL	35S-labeled	does not bind	NULL				deltaMEKK1	NULL		amino acids 1173-1493		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_16_13995_s_129	12584189	35S-Labeled GSK3beta bound to MEKK1-N1 (amino acids 1-401 of MEKK1) and MEKK1-N2 (amino acids 402-821) but not to MEKK1-deltaNC (amino acids 822-1172) or deltaMEKK1 (amino acids 1173-1493) (Fig.  5 A).	bind
32906	1	7906	5	13	NULL	NULL	NULL	Hairy protein	GP	35S-labeled	does not bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_17_17126_s_130	14871887	35S-Labeled Hairy protein was used as a control for the integrity of purified GST-proteins,  as Hairy did not bind GST ( lane 8), but could homodimerize ( lane 9) and heterodimerize with GST-E(spl)m3 ( lane 10), GST-E(spl)m8 ( lane 11), and GST-Deadpan ( lane 12).	bind
32907	2	7906	5	13	NULL	NULL	NULL	Hairy protein	GP	35S-labeled	homodimerize with					Hairy protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_17_17126_s_130	14871887	35S-Labeled Hairy protein was used as a control for the integrity of purified GST-proteins,  as Hairy did not bind GST ( lane 8), but could homodimerize ( lane 9) and heterodimerize with GST-E(spl)m3 ( lane 10), GST-E(spl)m8 ( lane 11), and GST-Deadpan ( lane 12).	bind
32908	3	7906	5	13	NULL	NULL	NULL	Hairy protein	GP	35S-labeled	heterodimerize with					GST-E(spl)m3	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_17_17126_s_130	14871887	35S-Labeled Hairy protein was used as a control for the integrity of purified GST-proteins,  as Hairy did not bind GST ( lane 8), but could homodimerize ( lane 9) and heterodimerize with GST-E(spl)m3 ( lane 10), GST-E(spl)m8 ( lane 11), and GST-Deadpan ( lane 12).	bind
32909	4	7906	5	13	NULL	NULL	NULL	Hairy protein	GP	35S-labeled	heterodimerize with					GST-E(spl)m8	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_17_17126_s_130	14871887	35S-Labeled Hairy protein was used as a control for the integrity of purified GST-proteins,  as Hairy did not bind GST ( lane 8), but could homodimerize ( lane 9) and heterodimerize with GST-E(spl)m3 ( lane 10), GST-E(spl)m8 ( lane 11), and GST-Deadpan ( lane 12).	bind
32910	5	7906	5	13	NULL	NULL	NULL	Hairy protein	GP	35S-labeled	heterodimerize with					GST-Deadpan	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_17_17126_s_130	14871887	35S-Labeled Hairy protein was used as a control for the integrity of purified GST-proteins,  as Hairy did not bind GST ( lane 8), but could homodimerize ( lane 9) and heterodimerize with GST-E(spl)m3 ( lane 10), GST-E(spl)m8 ( lane 11), and GST-Deadpan ( lane 12).	bind
25340	1	7906	6	10	NULL	0	NULL	Hairy protein		35S-Labeled	does not bind					GST					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_17_17126_s_130	14871887	35S-Labeled Hairy protein was used as a control for the integrity of purified GST-proteins,  as Hairy did not bind GST ( lane 8), but could homodimerize ( lane 9) and heterodimerize with GST-E(spl)m3 ( lane 10), GST-E(spl)m8 ( lane 11), and GST-Deadpan ( lane 12).	bind
25341	2	7906	6	10	NULL	0	NULL	Hairy protein		35S-Labeled	bind					Hairy protein					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_17_17126_s_130	14871887	35S-Labeled Hairy protein was used as a control for the integrity of purified GST-proteins,  as Hairy did not bind GST ( lane 8), but could homodimerize ( lane 9) and heterodimerize with GST-E(spl)m3 ( lane 10), GST-E(spl)m8 ( lane 11), and GST-Deadpan ( lane 12).	bind
25342	3	7906	6	10	NULL	0	NULL	Hairy protein		35S-Labeled	bind					GST-E(spl)m3					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_17_17126_s_130	14871887	35S-Labeled Hairy protein was used as a control for the integrity of purified GST-proteins,  as Hairy did not bind GST ( lane 8), but could homodimerize ( lane 9) and heterodimerize with GST-E(spl)m3 ( lane 10), GST-E(spl)m8 ( lane 11), and GST-Deadpan ( lane 12).	bind
25343	4	7906	6	10	NULL	0	NULL	Hairy protein		35S-Labeled	bind					GST-E(spl)m8					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_17_17126_s_130	14871887	35S-Labeled Hairy protein was used as a control for the integrity of purified GST-proteins,  as Hairy did not bind GST ( lane 8), but could homodimerize ( lane 9) and heterodimerize with GST-E(spl)m3 ( lane 10), GST-E(spl)m8 ( lane 11), and GST-Deadpan ( lane 12).	bind
25344	5	7906	6	10	NULL	0	NULL	Hairy protein		35S-Labeled	bind					GST-Deadpan					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_17_17126_s_130	14871887	35S-Labeled Hairy protein was used as a control for the integrity of purified GST-proteins,  as Hairy did not bind GST ( lane 8), but could homodimerize ( lane 9) and heterodimerize with GST-E(spl)m3 ( lane 10), GST-E(spl)m8 ( lane 11), and GST-Deadpan ( lane 12).	bind
32911	1	7907	5	13	NULL	NULL	NULL	HEF1	GP	35S-labeled	bind					GST-AIP4	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_28_29681_s_136	15051726	35S-Labeled HEF1 and Smad3 bound to GST-AIP4 were eluted from the beads, separated onto  SDS-PAGE, and detected by autoradiography.	bind
32912	2	7907	5	13	NULL	NULL	NULL	Smad3	GP	35S-labeled	bind					GST-AIP4	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_28_29681_s_136	15051726	35S-Labeled HEF1 and Smad3 bound to GST-AIP4 were eluted from the beads, separated onto  SDS-PAGE, and detected by autoradiography.	bind
25345	1	7907	6	NULL	NULL	0	NULL	HEF1	NULL	35S-labeled	bind	NULL				GST-AIP4	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_28_29681_s_136	15051726	35S-Labeled HEF1 and Smad3 bound to GST-AIP4 were eluted from the beads, separated onto  SDS-PAGE, and detected by autoradiography.	bind
25346	2	7907	6	NULL	NULL	0	NULL	Smad3	NULL	35S-labeled	bind	NULL				GST-AIP4	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_28_29681_s_136	15051726	35S-Labeled HEF1 and Smad3 bound to GST-AIP4 were eluted from the beads, separated onto  SDS-PAGE, and detected by autoradiography.	bind
32913	1	7908	5	13	NULL	NULL	NULL	INAD	GP	35S-labeled	bind					TRP GST fusion proteins	GP	wild-type	COOH-terminal 246 residues		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_150_6_1411_s_168	10995445	35S-labeled INAD bound to the GST fusion proteins consisting of the COOH-terminal 246 or 29 residues from wild-type TRP (referred to as long and short tails, respectively;   Fig 4A and   Fig B).	bind
32914	2	7908	5	13	NULL	NULL	NULL	INAD	GP	35S-labeled	bind					TRP GST fusion proteins	GP	wild-type	COOH-terminal 29 residues		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_150_6_1411_s_168	10995445	35S-labeled INAD bound to the GST fusion proteins consisting of the COOH-terminal 246 or 29 residues from wild-type TRP (referred to as long and short tails, respectively;   Fig 4A and   Fig B).	bind
32915	3	7908	5	13	NULL	NULL	NULL	statement 1	Process		is alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_150_6_1411_s_168	10995445	35S-labeled INAD bound to the GST fusion proteins consisting of the COOH-terminal 246 or 29 residues from wild-type TRP (referred to as long and short tails, respectively;   Fig 4A and   Fig B).	bind
25347	1	7908	6	NULL	NULL	0	NULL	INAD	NULL	35S-labeled	bind	NULL				TRP	NULL	wild type	COOH-terminal 246 residues		NULL		0	NULL	NULL	NULL	gw60_cellbiol_150_6_1411_s_168	10995445	35S-labeled INAD bound to the GST fusion proteins consisting of the COOH-terminal 246 or 29 residues from wild-type TRP (referred to as long and short tails, respectively;   Fig 4A and   Fig B).	bind
37306	2	7908	6	NULL	NULL	0	NULL	INAD	NULL	35S-labeled	bind	NULL				TRP	NULL	wild type	COOH-terminal 29 residues		NULL		0	NULL	NULL	NULL	gw60_cellbiol_150_6_1411_s_168	10995445	35S-labeled INAD bound to the GST fusion proteins consisting of the COOH-terminal 246 or 29 residues from wild-type TRP (referred to as long and short tails, respectively;   Fig 4A and   Fig B).	bind
47822	3	7908	6	10	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_150_6_1411_s_168	10995445	35S-labeled INAD bound to the GST fusion proteins consisting of the COOH-terminal 246 or 29 residues from wild-type TRP (referred to as long and short tails, respectively;   Fig 4A and   Fig B).	bind
32916	1	7909	5	13	NULL	NULL	NULL	Xsecurin	GP	35S-labeled;;IVT	bind					Cdc20	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_24_3278_s_113	11751633	35S-labeled IVT  Xsecurin was then added and the amount of securin bound to Cdc20 was analyzed as in  A and was quantitated on a PhosphorImager (graph).	bind
25348	1	7909	6	10	NULL	0	NULL	Xsecurin		35S-labeled;;IVT 	bind					Cdc20					NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_24_3278_s_113	11751633	35S-labeled IVT  Xsecurin was then added and the amount of securin bound to Cdc20 was analyzed as in  A and was quantitated on a PhosphorImager (graph).	bind
32917	1	7911	5	13	NULL	NULL	NULL	Mad2	GP	35S-labeled	bind					GST-Slp1	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_279_5353_1045_s_26	9461438	35S-labeled Mad2 bound to GST-Slp1, but not to GST (Fig.  1C).	bind
36181	2	7911	5	13	NULL	NULL	NULL	Mad2	GP	35S-labeled	does not bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_279_5353_1045_s_26	9461438	35S-labeled Mad2 bound to GST-Slp1, but not to GST (Fig.  1C).	bind
25350	1	7911	6	NULL	NULL	0	NULL	Mad2	NULL	35S-labeled	bind	NULL				GST-Slp1	NULL				NULL		0	NULL	NULL	NULL	gw60_science_279_5353_1045_s_26	9461438	35S-labeled Mad2 bound to GST-Slp1, but not to GST (Fig.  1C).	bind
25351	2	7911	6	NULL	NULL	0	NULL	Mad2	NULL	35S-labeled	does not bind	NULL				GST	NULL				NULL		0	NULL	NULL	NULL	gw60_science_279_5353_1045_s_26	9461438	35S-labeled Mad2 bound to GST-Slp1, but not to GST (Fig.  1C).	bind
32918	1	7912	5	13	NULL	NULL	NULL	MAN1	GP	35S-labeled	does not bind			N-terminus		emerin 	GP	mutant	delta95		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_14_13863_s_103	15681850	35S-Labeled MAN1-N did not bind the emerin mutant delta95 but recognized both lamin tails, particularly the B1 tail ( Fig. 3 B), independently confirming that MAN1 binds directly to both A- and B-type lamins.	bind
32919	2	7912	5	13	NULL	NULL	NULL	MAN1	GP	35S-labeled	bind			N-terminus		lamin	GP		B1 tail		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_14_13863_s_103	15681850	35S-Labeled MAN1-N did not bind the emerin mutant delta95 but recognized both lamin tails, particularly the B1 tail ( Fig. 3 B), independently confirming that MAN1 binds directly to both A- and B-type lamins.	bind
32920	3	7912	5	13	NULL	NULL	NULL	MAN1	GP		bind		directly			A-type lamins	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_14_13863_s_103	15681850	35S-Labeled MAN1-N did not bind the emerin mutant delta95 but recognized both lamin tails, particularly the B1 tail ( Fig. 3 B), independently confirming that MAN1 binds directly to both A- and B-type lamins.	bind
32921	4	7912	5	13	NULL	NULL	NULL	MAN1	GP		bind		directly			B-type lamins	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_14_13863_s_103	15681850	35S-Labeled MAN1-N did not bind the emerin mutant delta95 but recognized both lamin tails, particularly the B1 tail ( Fig. 3 B), independently confirming that MAN1 binds directly to both A- and B-type lamins.	bind
25352	1	7912	6	NULL	NULL	0	NULL	MAN1	NULL	35S-labeled	does not bind	NULL		N-terminus		emerin	NULL	mutant	delta95		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_14_13863_s_103	15681850	35S-Labeled MAN1-N did not bind the emerin mutant delta95 but recognized both lamin tails, particularly the B1 tail ( Fig. 3 B), independently confirming that MAN1 binds directly to both A- and B-type lamins.	bind
25353	2	7912	6	10	NULL	0	NULL	MAN1			bind		directly			A-type lamins					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_14_13863_s_103	15681850	35S-Labeled MAN1-N did not bind the emerin mutant delta95 but recognized both lamin tails, particularly the B1 tail ( Fig. 3 B), independently confirming that MAN1 binds directly to both A- and B-type lamins.	bind
25354	3	7912	6	10	NULL	0	NULL	MAN1			bind		directly			B-type lamins					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_14_13863_s_103	15681850	35S-Labeled MAN1-N did not bind the emerin mutant delta95 but recognized both lamin tails, particularly the B1 tail ( Fig. 3 B), independently confirming that MAN1 binds directly to both A- and B-type lamins.	bind
47823	4	7912	6	10	NULL	0	NULL	MAN1		35S-labeled	bind			N-terminus		lamin			B1 tail		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_14_13863_s_103	15681850	35S-Labeled MAN1-N did not bind the emerin mutant delta95 but recognized both lamin tails, particularly the B1 tail ( Fig. 3 B), independently confirming that MAN1 binds directly to both A- and B-type lamins.	bind
32922	1	7914	5	13	NULL	NULL	NULL	p150Glued	GP	35S-labeled	does not bind					betaIII spectrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_39_36598_s_94	11461920	35S-labeled p150Glued did not bind to either the betaIII spectrin column or the GST column.	bind
32923	2	7914	5	13	NULL	NULL	NULL	p150Glued	GP	35S-labeled	does not bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_39_36598_s_94	11461920	35S-labeled p150Glued did not bind to either the betaIII spectrin column or the GST column.	bind
25357	1	7914	6	NULL	NULL	0	NULL	p150Glued	NULL	35S-labeled	does not bind	NULL				betaIII spectrin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_39_36598_s_94	11461920	35S-labeled p150Glued did not bind to either the betaIII spectrin column or the GST column.	bind
25358	2	7914	6	NULL	NULL	0	NULL	p150Glued	NULL	35S-labeled	does not bind	NULL				GST column	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_39_36598_s_94	11461920	35S-labeled p150Glued did not bind to either the betaIII spectrin column or the GST column.	bind
32924	1	7922	5	13	NULL	NULL	NULL	RpS21 protein	GP	35S-labeled	bind					GST-P40	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_2308_s_331	10022917	35S-labeled RpS21 proteins bound to GST-P40 (lane 1) or GST proteins (lane 2) were analyzed by SDS-PAGE and detected by autoradiography.	bind
25359	1	7922	6	NULL	NULL	0	NULL	RpS21 protein	NULL	35S-labeled	bind	NULL				GST-P40	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_3_2308_s_331	10022917	35S-labeled RpS21 proteins bound to GST-P40 (lane 1) or GST proteins (lane 2) were analyzed by SDS-PAGE and detected by autoradiography.	bind
32925	1	7923	5	13	NULL	NULL	NULL	SFV	GP	35S-labeled	bind					BHK cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_1_111_s_190	16216925	35S-labeled SFV was bound to BHK cells on ice and treated at pH 7.4 or 5.5 at 37 degrees  C for 1 min in the presence of the indicated domain III proteins.	bind
32926	2	7923	5	13	NULL	NULL	NULL	statement 1	Process		in presence of					domain III proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_1_111_s_190	16216925	35S-labeled SFV was bound to BHK cells on ice and treated at pH 7.4 or 5.5 at 37 degrees  C for 1 min in the presence of the indicated domain III proteins.	bind
25360	1	7923	6	NULL	NULL	0	NULL	SFV	NULL	35S-labeled	bind	NULL				BHK cells	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_171_1_111_s_190	16216925	35S-labeled SFV was bound to BHK cells on ice and treated at pH 7.4 or 5.5 at 37 degrees  C for 1 min in the presence of the indicated domain III proteins.	bind
47824	2	7923	6	10	NULL	0	NULL	statement 1	NULL		in presence of	NULL				domain III proteins	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_171_1_111_s_190	16216925	35S-labeled SFV was bound to BHK cells on ice and treated at pH 7.4 or 5.5 at 37 degrees  C for 1 min in the presence of the indicated domain III proteins.	bind
32927	1	7924	5	13	NULL	NULL	NULL	Smad3	GP	35S-labeled	bind					GST-AIP4	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_28_29681_s_155	15051726	35S-Labeled Smad3 and HEF1 were found to bind GST-AIP4 ( Fig. 1 D,  lanes 3 and  4).	bind
32928	2	7924	5	13	NULL	NULL	NULL	HEF1	GP	35S-labeled	bind					GST-AIP4	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_28_29681_s_155	15051726	35S-Labeled Smad3 and HEF1 were found to bind GST-AIP4 ( Fig. 1 D,  lanes 3 and  4).	bind
25361	1	7924	6	NULL	NULL	0	NULL	Smad3	NULL	35S-labeled	bind	NULL				GST-AIP4	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_28_29681_s_155	15051726	35S-Labeled Smad3 and HEF1 were found to bind GST-AIP4 ( Fig. 1 D,  lanes 3 and  4).	bind
25362	2	7924	6	NULL	NULL	0	NULL	HEF1	NULL	35S-labeled	bind	NULL				GST-AIP4	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_28_29681_s_155	15051726	35S-Labeled Smad3 and HEF1 were found to bind GST-AIP4 ( Fig. 1 D,  lanes 3 and  4).	bind
32929	1	7925	5	13	NULL	NULL	NULL	SR1-5	GP	35S-labeled	bind		specifically			GST-SR5-6	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_525_1_135_s_81	12163176	35S-labeled SR1-5 also bound specifically to GST-SR5-6 on GST-sepharose columns (data not shown).	bind
25363	1	7925	6	NULL	NULL	0	NULL	SR1-5	NULL	35 S-labeled	bind	NULL	specifically			GST-SR5-6	NULL				NULL		NULL	NULL	NULL	NULL	gw60_febslett_525_1_135_s_81	12163176	35S-labeled SR1-5 also bound specifically to GST-SR5-6 on GST-sepharose columns (data not shown).	bind
32930	1	7926	5	13	NULL	NULL	NULL	SR2-3	GP	35S-labeled	bind					GST-SR5-6	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_525_1_135_s_84	12163176	35S-labeled SR2-3 and SR3 each bound to GST-SR5-6 ( Fig. 2D,F), but SR2 did not (  Fig. 2E), suggesting that SR3 is sufficient to bind SR5-6.	bind
32931	2	7926	5	13	NULL	NULL	NULL	SR3	GP	35S-labeled	bind					GST-SR5-6	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_525_1_135_s_84	12163176	35S-labeled SR2-3 and SR3 each bound to GST-SR5-6 ( Fig. 2D,F), but SR2 did not (  Fig. 2E), suggesting that SR3 is sufficient to bind SR5-6.	bind
32932	3	7926	5	13	NULL	NULL	NULL	SR2	GP	35S-labeled	does not bind					GST-SR5-6	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_525_1_135_s_84	12163176	35S-labeled SR2-3 and SR3 each bound to GST-SR5-6 ( Fig. 2D,F), but SR2 did not (  Fig. 2E), suggesting that SR3 is sufficient to bind SR5-6.	bind
32933	4	7926	5	13	NULL	NULL	NULL	SR3	GP	35S-labeled	bind					SR5-6	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_525_1_135_s_84	12163176	35S-labeled SR2-3 and SR3 each bound to GST-SR5-6 ( Fig. 2D,F), but SR2 did not (  Fig. 2E), suggesting that SR3 is sufficient to bind SR5-6.	bind
36178	5	7926	5	13	NULL	NULL	NULL	statement 1	Process		suggest					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_525_1_135_s_84	12163176	35S-labeled SR2-3 and SR3 each bound to GST-SR5-6 ( Fig. 2D,F), but SR2 did not (  Fig. 2E), suggesting that SR3 is sufficient to bind SR5-6.	bind
36179	6	7926	5	13	NULL	NULL	NULL	statement 2	Process		suggest					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_525_1_135_s_84	12163176	35S-labeled SR2-3 and SR3 each bound to GST-SR5-6 ( Fig. 2D,F), but SR2 did not (  Fig. 2E), suggesting that SR3 is sufficient to bind SR5-6.	bind
36180	7	7926	5	13	NULL	NULL	NULL	statement 3	Process		suggest					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_525_1_135_s_84	12163176	35S-labeled SR2-3 and SR3 each bound to GST-SR5-6 ( Fig. 2D,F), but SR2 did not (  Fig. 2E), suggesting that SR3 is sufficient to bind SR5-6.	bind
25365	1	7926	6	10	NULL	0	NULL	SR2-3		35S-labeled	bind					GST-SR5-6					NULL		NULL	NULL	NULL	NULL	gw60_febslett_525_1_135_s_84	12163176	35S-labeled SR2-3 and SR3 each bound to GST-SR5-6 ( Fig. 2D,F), but SR2 did not (  Fig. 2E), suggesting that SR3 is sufficient to bind SR5-6.	bind
25366	2	7926	6	10	NULL	0	NULL	SR3		35S-labeled	bind					GST-SR5-6					NULL		NULL	NULL	NULL	NULL	gw60_febslett_525_1_135_s_84	12163176	35S-labeled SR2-3 and SR3 each bound to GST-SR5-6 ( Fig. 2D,F), but SR2 did not (  Fig. 2E), suggesting that SR3 is sufficient to bind SR5-6.	bind
25367	3	7926	6	10	NULL	0	NULL	SR2		35S-labeled	does not bind					GST-SR5-6					NULL		NULL	NULL	NULL	NULL	gw60_febslett_525_1_135_s_84	12163176	35S-labeled SR2-3 and SR3 each bound to GST-SR5-6 ( Fig. 2D,F), but SR2 did not (  Fig. 2E), suggesting that SR3 is sufficient to bind SR5-6.	bind
37307	4	7926	6	10	NULL	0	NULL	SR3		35S-labeled	bind					SR5-6					NULL		NULL	NULL	NULL	NULL	gw60_febslett_525_1_135_s_84	12163176	35S-labeled SR2-3 and SR3 each bound to GST-SR5-6 ( Fig. 2D,F), but SR2 did not (  Fig. 2E), suggesting that SR3 is sufficient to bind SR5-6.	bind
37308	5	7926	6	NULL	NULL	0	NULL	statement 1	NULL		suggests	NULL				statement 4	NULL				NULL		NULL	NULL	NULL	NULL	gw60_febslett_525_1_135_s_84	12163176	35S-labeled SR2-3 and SR3 each bound to GST-SR5-6 ( Fig. 2D,F), but SR2 did not (  Fig. 2E), suggesting that SR3 is sufficient to bind SR5-6.	bind
37309	6	7926	6	NULL	NULL	0	NULL	statement 2	NULL		suggests	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_525_1_135_s_84	12163176	35S-labeled SR2-3 and SR3 each bound to GST-SR5-6 ( Fig. 2D,F), but SR2 did not (  Fig. 2E), suggesting that SR3 is sufficient to bind SR5-6.	bind
37310	7	7926	6	NULL	NULL	0	NULL	statement 3	NULL		suggests	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_525_1_135_s_84	12163176	35S-labeled SR2-3 and SR3 each bound to GST-SR5-6 ( Fig. 2D,F), but SR2 did not (  Fig. 2E), suggesting that SR3 is sufficient to bind SR5-6.	bind
32934	1	7931	5	13	NULL	NULL	NULL	HIRA	GP	35S-labeled	bind					GST-HIRIP5	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1517_3_376_s_66	11342215	35S-labelled HIRA (arrow) binds GST-HIRIP5 but not GST immobilized on glutathione beads.	bind
32935	2	7931	5	13	NULL	NULL	NULL	HIRA	GP	35S-labeled	does not bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1517_3_376_s_66	11342215	35S-labelled HIRA (arrow) binds GST-HIRIP5 but not GST immobilized on glutathione beads.	bind
25368	1	7931	6	NULL	NULL	0	NULL	HIRA	NULL	35S-labeled	bind	NULL				GST-HIRIP5	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1517_3_376_s_66	11342215	35S-labelled HIRA (arrow) binds GST-HIRIP5 but not GST immobilized on glutathione beads.	bind
25369	2	7931	6	NULL	NULL	0	NULL	HIRA	NULL	35S-labeled	does not bind	NULL				GST	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1517_3_376_s_66	11342215	35S-labelled HIRA (arrow) binds GST-HIRIP5 but not GST immobilized on glutathione beads.	bind
32936	1	7933	5	13	NULL	NULL	NULL	IB1	GP	35S-radiolabeled;;full-length	bind					IB1	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_785_s_50	16456539	35S-radiolabeled full-length IB1 was found to bind to the SH3 domains of IB1 and to  a weaker extent to that of IB2, but neither to GST alone nor to the GAP or Grb2 SH3  domains ( Figure 2A).	bind
32937	2	7933	5	13	NULL	NULL	NULL	IB1	GP	35S-radiolabeled;;full-length	bind		weakly			IB2	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_785_s_50	16456539	35S-radiolabeled full-length IB1 was found to bind to the SH3 domains of IB1 and to  a weaker extent to that of IB2, but neither to GST alone nor to the GAP or Grb2 SH3  domains ( Figure 2A).	bind
32938	3	7933	5	13	NULL	NULL	NULL	IB1	GP	35S-radiolabeled;;full-length	does not bind					GST	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_785_s_50	16456539	35S-radiolabeled full-length IB1 was found to bind to the SH3 domains of IB1 and to  a weaker extent to that of IB2, but neither to GST alone nor to the GAP or Grb2 SH3  domains ( Figure 2A).	bind
32939	4	7933	5	13	NULL	NULL	NULL	IB1	GP	35S-radiolabeled;;full-length	does not bind					GAP	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_785_s_50	16456539	35S-radiolabeled full-length IB1 was found to bind to the SH3 domains of IB1 and to  a weaker extent to that of IB2, but neither to GST alone nor to the GAP or Grb2 SH3  domains ( Figure 2A).	bind
32940	5	7933	5	13	NULL	NULL	NULL	IB1	GP	35S-radiolabeled;;full-length	does not bind					Grb2	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_785_s_50	16456539	35S-radiolabeled full-length IB1 was found to bind to the SH3 domains of IB1 and to  a weaker extent to that of IB2, but neither to GST alone nor to the GAP or Grb2 SH3  domains ( Figure 2A).	bind
25370	1	7933	6	10	NULL	0	NULL	IB1	NULL	35S-radiolabeled;;full-length 	bind	NULL				IB1	NULL		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_785_s_50	16456539	35S-radiolabeled full-length IB1 was found to bind to the SH3 domains of IB1 and to  a weaker extent to that of IB2, but neither to GST alone nor to the GAP or Grb2 SH3  domains ( Figure 2A).	bind
25371	2	7933	6	10	NULL	0	NULL	IB1	NULL	35S-radiolabeled;;full-length 	bind	NULL	weakly			IB2	NULL		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_785_s_50	16456539	35S-radiolabeled full-length IB1 was found to bind to the SH3 domains of IB1 and to  a weaker extent to that of IB2, but neither to GST alone nor to the GAP or Grb2 SH3  domains ( Figure 2A).	bind
25372	3	7933	6	10	NULL	0	NULL	IB1	NULL	35S-radiolabeled;;full-length 	does not bind	NULL				GAP	NULL		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_785_s_50	16456539	35S-radiolabeled full-length IB1 was found to bind to the SH3 domains of IB1 and to  a weaker extent to that of IB2, but neither to GST alone nor to the GAP or Grb2 SH3  domains ( Figure 2A).	bind
25373	4	7933	6	10	NULL	0	NULL	IB1	NULL	35S-radiolabeled;;full-length 	does not bind	NULL				Grb2	NULL		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_4_785_s_50	16456539	35S-radiolabeled full-length IB1 was found to bind to the SH3 domains of IB1 and to  a weaker extent to that of IB2, but neither to GST alone nor to the GAP or Grb2 SH3  domains ( Figure 2A).	bind
32941	2	7934	5	13	NULL	NULL	NULL	35S-Stbm	GP		defines			CtermdeltaC2					85 amino acids region		NULL		NULL	NULL	NULL	NULL	gw70_development_131_18_4467_s_247	15306567	35S-Stbm CtermdeltaN2 and 35S-Stbm CtermdeltaC2 define a region of 85 amino acids required for binding of Stbm to Dgo.	bind
32942	3	7934	5	13	NULL	NULL	NULL	Stbm	GP		bind					Dgo	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_131_18_4467_s_247	15306567	35S-Stbm CtermdeltaN2 and 35S-Stbm CtermdeltaC2 define a region of 85 amino acids required for binding of Stbm to Dgo.	bind
32943	4	7934	5	13	NULL	NULL	NULL	statement 1	Process		is required for					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_131_18_4467_s_247	15306567	35S-Stbm CtermdeltaN2 and 35S-Stbm CtermdeltaC2 define a region of 85 amino acids required for binding of Stbm to Dgo.	bind
32944	1	7934	5	13	NULL	NULL	NULL	35S-Stbm	GP		defines			CtermdeltaN2					85 amino acids region		NULL		NULL	NULL	NULL	NULL	gw70_development_131_18_4467_s_247	15306567	35S-Stbm CtermdeltaN2 and 35S-Stbm CtermdeltaC2 define a region of 85 amino acids required for binding of Stbm to Dgo.	bind
47825	5	7934	5	13	NULL	NULL	NULL	statement 2	Process		is required for					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_131_18_4467_s_247	15306567	35S-Stbm CtermdeltaN2 and 35S-Stbm CtermdeltaC2 define a region of 85 amino acids required for binding of Stbm to Dgo.	bind
25742	1	7934	6	NULL	NULL	0	NULL	Stbm	NULL		bind	NULL				Dgo	NULL				NULL		0	NULL	NULL	NULL	gw70_development_131_18_4467_s_247	15306567	35S-Stbm CtermdeltaN2 and 35S-Stbm CtermdeltaC2 define a region of 85 amino acids required for binding of Stbm to Dgo.	bind
25743	2	7934	6	NULL	NULL	0	NULL	Stbm	NULL		is required for	NULL		CtermdeltaN2		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_development_131_18_4467_s_247	15306567	35S-Stbm CtermdeltaN2 and 35S-Stbm CtermdeltaC2 define a region of 85 amino acids required for binding of Stbm to Dgo.	bind
25744	3	7934	6	NULL	NULL	0	NULL	Stbm	NULL		is required for	NULL		CtermdeltaC2		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_development_131_18_4467_s_247	15306567	35S-Stbm CtermdeltaN2 and 35S-Stbm CtermdeltaC2 define a region of 85 amino acids required for binding of Stbm to Dgo.	bind
47826	4	7934	6	10	NULL	0	NULL	35S-Stbm	NULL		defines	NULL		CtermdeltaC2		85 amino acid region	NULL				NULL		0	NULL	NULL	NULL	gw70_development_131_18_4467_s_247	15306567	35S-Stbm CtermdeltaN2 and 35S-Stbm CtermdeltaC2 define a region of 85 amino acids required for binding of Stbm to Dgo.	bind
47827	5	7934	6	10	NULL	0	NULL	35S-Stbm	NULL		defines	NULL		CtermdeltaN2		85 amino acid region	NULL				NULL		0	NULL	NULL	NULL	gw70_development_131_18_4467_s_247	15306567	35S-Stbm CtermdeltaN2 and 35S-Stbm CtermdeltaC2 define a region of 85 amino acids required for binding of Stbm to Dgo.	bind
32945	1	7936	5	13	NULL	NULL	NULL	Zinc(II) ions	Chemical		interacts with		selectively			5S-RNA gene	GP	Xenopus		DNA sequences at TFIIIA binding site	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2772_s_381	11433022	36       Martinez-Balbas,M.A., Jimenez-Garcia,E. and Azorin,F. (1995) Zinc(II) ions selectively interact with DNA sequences present at the TFIIIA binding site of the  Xenopus 5S-RNA gene.	bind
25494	1	7936	6	NULL	NULL	0	NULL	Zinc(II) ions	NULL		interact with	NULL	selectively			5S-RNA gene	NULL	Xenopus		TFIIIA binding site 	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2772_s_381	11433022	36       Martinez-Balbas,M.A., Jimenez-Garcia,E. and Azorin,F. (1995) Zinc(II) ions selectively interact with DNA sequences present at the TFIIIA binding site of the  Xenopus 5S-RNA gene.	bind
32946	1	7937	5	13	NULL	NULL	NULL	c-myb proto-oncogene product	GP		bind									simian virus 40 enhancer	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_17_3546_s_453	11522824	36       Nakagoshi,H., Nagase,T., Kanei-Ishii,C., Ueno,Y. and Ishii,S. (1990) Binding of the c-myb proto-oncogene product to the simian virus 40 enhancer stimulates transcription.	bind
32947	2	7937	5	13	NULL	NULL	NULL	statement 1	Process		stimulates					transcription	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_17_3546_s_453	11522824	36       Nakagoshi,H., Nagase,T., Kanei-Ishii,C., Ueno,Y. and Ishii,S. (1990) Binding of the c-myb proto-oncogene product to the simian virus 40 enhancer stimulates transcription.	bind
25495	1	7937	6	NULL	NULL	0	NULL	c-myb proto-oncogene	NULL		bind	NULL					NULL			simian virus 40 enhancer	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_17_3546_s_453	11522824	36       Nakagoshi,H., Nagase,T., Kanei-Ishii,C., Ueno,Y. and Ishii,S. (1990) Binding of the c-myb proto-oncogene product to the simian virus 40 enhancer stimulates transcription.	bind
25497	2	7937	6	NULL	NULL	0	NULL	statement 1	NULL		stimulates	NULL				transcription	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_17_3546_s_453	11522824	36       Nakagoshi,H., Nagase,T., Kanei-Ishii,C., Ueno,Y. and Ishii,S. (1990) Binding of the c-myb proto-oncogene product to the simian virus 40 enhancer stimulates transcription.	bind
32948	1	7938	5	13	NULL	NULL	NULL	Poly (rC) binding protein 2	GP		forms ternary complex with					poliovirus RNA	NucleicAcid			5''-terminal sequences	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2715_s_499	11433016	36       Parsley,T.B., Towner,J.S., Blyn,L.B., Ehrenfeld,E. and Semler,B.L. (1997) Poly (rC) binding protein 2 forms a ternary complex with the 5''-terminal sequences of poliovirus RNA and the viral 3CD proteinase.	bind
32949	2	7938	5	13	NULL	NULL	NULL	Poly (rC) binding protein 2	GP		forms ternary complex with					3CD proteinase	GP	viral			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2715_s_499	11433016	36       Parsley,T.B., Towner,J.S., Blyn,L.B., Ehrenfeld,E. and Semler,B.L. (1997) Poly (rC) binding protein 2 forms a ternary complex with the 5''-terminal sequences of poliovirus RNA and the viral 3CD proteinase.	bind
37891	3	7938	5	13	NULL	NULL	NULL	statement 1	Process		occurs simultaneously with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2715_s_499	11433016	36       Parsley,T.B., Towner,J.S., Blyn,L.B., Ehrenfeld,E. and Semler,B.L. (1997) Poly (rC) binding protein 2 forms a ternary complex with the 5''-terminal sequences of poliovirus RNA and the viral 3CD proteinase.	bind
25740	1	7938	6	NULL	NULL	0	NULL	Poly (rC) binding protein 2	NULL		forms ternary complex with	NULL				poliovirus RNA	NULL			5''-terminal sequences	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2715_s_499	11433016	36       Parsley,T.B., Towner,J.S., Blyn,L.B., Ehrenfeld,E. and Semler,B.L. (1997) Poly (rC) binding protein 2 forms a ternary complex with the 5''-terminal sequences of poliovirus RNA and the viral 3CD proteinase.	bind
25741	2	7938	6	NULL	NULL	0	NULL	Poly (rC) binding protein 2	NULL		forms a ternary complex with	NULL				3CD proteinase	NULL	viral			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2715_s_499	11433016	36       Parsley,T.B., Towner,J.S., Blyn,L.B., Ehrenfeld,E. and Semler,B.L. (1997) Poly (rC) binding protein 2 forms a ternary complex with the 5''-terminal sequences of poliovirus RNA and the viral 3CD proteinase.	bind
37880	3	7938	6	NULL	NULL	0	NULL	statement 1	NULL		occurs simultaneously with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2715_s_499	11433016	36       Parsley,T.B., Towner,J.S., Blyn,L.B., Ehrenfeld,E. and Semler,B.L. (1997) Poly (rC) binding protein 2 forms a ternary complex with the 5''-terminal sequences of poliovirus RNA and the viral 3CD proteinase.	bind
32950	1	7939	5	13	NULL	NULL	NULL	Cu2+	Chemical		bind					LDL	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3338_s_54	9409331	36  37  To investigate the possible role of histidine residues in the binding of Cu2+ to LDL and the resulting peroxidation of LDL lipid, we used DEPC to modify this amino acid.	bind
32953	2	7939	5	13	NULL	NULL	NULL	histidine residues	AminoAcid		plays a role in		possibly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3338_s_54	9409331	36  37  To investigate the possible role of histidine residues in the binding of Cu2+ to LDL and the resulting peroxidation of LDL lipid, we used DEPC to modify this amino acid.	bind
32954	3	7939	5	13	NULL	NULL	NULL	statement 2	Process		results in					LDL lipid	Chemical	peroxidation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3338_s_54	9409331	36  37  To investigate the possible role of histidine residues in the binding of Cu2+ to LDL and the resulting peroxidation of LDL lipid, we used DEPC to modify this amino acid.	bind
25498	1	7939	6	NULL	NULL	0	NULL	Cu2+	NULL		bind	NULL				LDL	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3338_s_54	9409331	36  37  To investigate the possible role of histidine residues in the binding of Cu2+ to LDL and the resulting peroxidation of LDL lipid, we used DEPC to modify this amino acid.	bind
37311	2	7939	6	NULL	NULL	0	NULL	histidine residues	NULL		plays a role in	NULL	possibly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3338_s_54	9409331	36  37  To investigate the possible role of histidine residues in the binding of Cu2+ to LDL and the resulting peroxidation of LDL lipid, we used DEPC to modify this amino acid.	bind
37312	3	7939	6	NULL	NULL	0	NULL	statement 2	NULL		results in	NULL				LDL lipid	NULL	peroxidation of 			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_3338_s_54	9409331	36  37  To investigate the possible role of histidine residues in the binding of Cu2+ to LDL and the resulting peroxidation of LDL lipid, we used DEPC to modify this amino acid.	bind
32955	1	7940	5	13	NULL	NULL	NULL	bFGF	GP	active	bind					HS	Chemical				NULL	lumenal surface of blood vessels	NULL	NULL	NULL	NULL	gw60_circulation_95_7_1853_s_234	9107173	36  41 42  The present study raises the possibility that in spite of its antiproliferative effect, heparin may also exert an undesirable effect, ie, displacement of active bFGF that is normally bound to HS on the lumenal surface of blood vessels.	bind
32956	2	7940	5	13	NULL	NULL	NULL	heparin	Chemical		displace					bFGF	GP	active			NULL	lumenal surface of blood vessels	NULL	NULL	NULL	NULL	gw60_circulation_95_7_1853_s_234	9107173	36  41 42  The present study raises the possibility that in spite of its antiproliferative effect, heparin may also exert an undesirable effect, ie, displacement of active bFGF that is normally bound to HS on the lumenal surface of blood vessels.	bind
25510	1	7940	6	NULL	NULL	0	NULL	bFGF	NULL	active	bind	NULL	normally			HS	NULL				NULL	lumenal surface of blood vessels	NULL	NULL	NULL	NULL	gw60_circulation_95_7_1853_s_234	9107173	36  41 42  The present study raises the possibility that in spite of its antiproliferative effect, heparin may also exert an undesirable effect, ie, displacement of active bFGF that is normally bound to HS on the lumenal surface of blood vessels.	bind
25511	2	7940	6	NULL	NULL	0	NULL	heparin	NULL		displaces	NULL				bFGF	NULL	active			NULL	lumenal surface of blood vessels	NULL	NULL	NULL	NULL	gw60_circulation_95_7_1853_s_234	9107173	36  41 42  The present study raises the possibility that in spite of its antiproliferative effect, heparin may also exert an undesirable effect, ie, displacement of active bFGF that is normally bound to HS on the lumenal surface of blood vessels.	bind
32957	1	7941	5	13	NULL	NULL	NULL	SRF	GP		bind									A/T-rich DNA sequence	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_2_188_s_193	8575061	36  SRF binds an A/T-rich DNA sequence, referred to as the serum response element, or CArG box.	bind
32958	2	7941	5	13	NULL	NULL	NULL	A/T-rich DNA sequence	NucleicAcid		referred to as					serum response element	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_2_188_s_193	8575061	36  SRF binds an A/T-rich DNA sequence, referred to as the serum response element, or CArG box.	bind
32959	3	7941	5	13	NULL	NULL	NULL	A/T-rich DNA sequence	NucleicAcid		referred to as					CArG box	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_2_188_s_193	8575061	36  SRF binds an A/T-rich DNA sequence, referred to as the serum response element, or CArG box.	bind
32960	4	7941	5	13	NULL	NULL	NULL	statement 2	Process		is alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_2_188_s_193	8575061	36  SRF binds an A/T-rich DNA sequence, referred to as the serum response element, or CArG box.	bind
25512	1	7941	6	10	NULL	0	NULL	A/T-rich DNA sequence	NULL		referred as	NULL				serum response element	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_2_188_s_193	8575061	36  SRF binds an A/T-rich DNA sequence, referred to as the serum response element, or CArG box.	bind
25513	2	7941	6	NULL	NULL	0	NULL	SRF	NULL		bind	NULL					NULL			A/T-rich DNA sequence	NULL		0	NULL	NULL	NULL	gw60_circulationres_78_2_188_s_193	8575061	36  SRF binds an A/T-rich DNA sequence, referred to as the serum response element, or CArG box.	bind
47828	3	7941	6	10	NULL	0	NULL	A/T-rich DNA sequence	NULL		referred as	NULL				CArG box	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_78_2_188_s_193	8575061	36  SRF binds an A/T-rich DNA sequence, referred to as the serum response element, or CArG box.	bind
47830	4	7941	6	10	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_78_2_188_s_193	8575061	36  SRF binds an A/T-rich DNA sequence, referred to as the serum response element, or CArG box.	bind
32961	1	7942	5	13	NULL	NULL	NULL	platelet glycoprotein Ia/IIa	GP		bind					collagen	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_8_1128_s_141	11222477	36  The reactions of platelets are mostly integrin-dependent, involving the binding of platelet glycoprotein Ia/IIa to collagen and glycoprotein IIb/IIa to fibrinogen, which results in shape change, release of granule contents, and aggregation, leading to thrombus growth at the sites of arterial injury.	bind
32962	2	7942	5	13	NULL	NULL	NULL	glycoprotein IIb/IIa	GP		bind					fibrinogen	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_8_1128_s_141	11222477	36  The reactions of platelets are mostly integrin-dependent, involving the binding of platelet glycoprotein Ia/IIa to collagen and glycoprotein IIb/IIa to fibrinogen, which results in shape change, release of granule contents, and aggregation, leading to thrombus growth at the sites of arterial injury.	bind
32963	3	7942	5	13	NULL	NULL	NULL	statement 1	Process		is dependent on					integrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_8_1128_s_141	11222477	36  The reactions of platelets are mostly integrin-dependent, involving the binding of platelet glycoprotein Ia/IIa to collagen and glycoprotein IIb/IIa to fibrinogen, which results in shape change, release of granule contents, and aggregation, leading to thrombus growth at the sites of arterial injury.	bind
32964	4	7942	5	13	NULL	NULL	NULL	statement 2	Process		is dependent on					integrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_8_1128_s_141	11222477	36  The reactions of platelets are mostly integrin-dependent, involving the binding of platelet glycoprotein Ia/IIa to collagen and glycoprotein IIb/IIa to fibrinogen, which results in shape change, release of granule contents, and aggregation, leading to thrombus growth at the sites of arterial injury.	bind
32965	5	7942	5	13	NULL	NULL	NULL	statement 1	Process		results in					shape	Process	change of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_8_1128_s_141	11222477	36  The reactions of platelets are mostly integrin-dependent, involving the binding of platelet glycoprotein Ia/IIa to collagen and glycoprotein IIb/IIa to fibrinogen, which results in shape change, release of granule contents, and aggregation, leading to thrombus growth at the sites of arterial injury.	bind
32966	6	7942	5	13	NULL	NULL	NULL	statement 1	Process		results in					granule contents	Process	release of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_8_1128_s_141	11222477	36  The reactions of platelets are mostly integrin-dependent, involving the binding of platelet glycoprotein Ia/IIa to collagen and glycoprotein IIb/IIa to fibrinogen, which results in shape change, release of granule contents, and aggregation, leading to thrombus growth at the sites of arterial injury.	bind
32967	7	7942	5	13	NULL	NULL	NULL	statement 1	Process		results in					aggregation	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_8_1128_s_141	11222477	36  The reactions of platelets are mostly integrin-dependent, involving the binding of platelet glycoprotein Ia/IIa to collagen and glycoprotein IIb/IIa to fibrinogen, which results in shape change, release of granule contents, and aggregation, leading to thrombus growth at the sites of arterial injury.	bind
32968	8	7942	5	13	NULL	NULL	NULL	statement 5	Process		leads to					thrombus	Process	growth of			NULL	at the sites of arterial injury	NULL	NULL	NULL	NULL	gw60_circulation_103_8_1128_s_141	11222477	36  The reactions of platelets are mostly integrin-dependent, involving the binding of platelet glycoprotein Ia/IIa to collagen and glycoprotein IIb/IIa to fibrinogen, which results in shape change, release of granule contents, and aggregation, leading to thrombus growth at the sites of arterial injury.	bind
32969	9	7942	5	13	NULL	NULL	NULL	statement 6	Process		leads to					thrombus	Process	growth of			NULL	at the sites of arterial injury	NULL	NULL	NULL	NULL	gw60_circulation_103_8_1128_s_141	11222477	36  The reactions of platelets are mostly integrin-dependent, involving the binding of platelet glycoprotein Ia/IIa to collagen and glycoprotein IIb/IIa to fibrinogen, which results in shape change, release of granule contents, and aggregation, leading to thrombus growth at the sites of arterial injury.	bind
32970	10	7942	5	13	NULL	NULL	NULL	statement 7	Process		leads to					thrombus	Process	growth of			NULL	at the sites of arterial injury	NULL	NULL	NULL	NULL	gw60_circulation_103_8_1128_s_141	11222477	36  The reactions of platelets are mostly integrin-dependent, involving the binding of platelet glycoprotein Ia/IIa to collagen and glycoprotein IIb/IIa to fibrinogen, which results in shape change, release of granule contents, and aggregation, leading to thrombus growth at the sites of arterial injury.	bind
32971	11	7942	5	13	NULL	NULL	NULL	statement 2	Process		results in					shape	Process	change of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_8_1128_s_141	11222477	36  The reactions of platelets are mostly integrin-dependent, involving the binding of platelet glycoprotein Ia/IIa to collagen and glycoprotein IIb/IIa to fibrinogen, which results in shape change, release of granule contents, and aggregation, leading to thrombus growth at the sites of arterial injury.	bind
32972	12	7942	5	13	NULL	NULL	NULL	statement 2	Process		results in					granule contents	Process	release of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_8_1128_s_141	11222477	36  The reactions of platelets are mostly integrin-dependent, involving the binding of platelet glycoprotein Ia/IIa to collagen and glycoprotein IIb/IIa to fibrinogen, which results in shape change, release of granule contents, and aggregation, leading to thrombus growth at the sites of arterial injury.	bind
32974	14	7942	5	13	NULL	NULL	NULL	statement 11	Process		leads to					thrombus	Process	growth of			NULL	at the sites of arterial injury	NULL	NULL	NULL	NULL	gw60_circulation_103_8_1128_s_141	11222477	36  The reactions of platelets are mostly integrin-dependent, involving the binding of platelet glycoprotein Ia/IIa to collagen and glycoprotein IIb/IIa to fibrinogen, which results in shape change, release of granule contents, and aggregation, leading to thrombus growth at the sites of arterial injury.	bind
32975	15	7942	5	13	NULL	NULL	NULL	statement 12	Process		leads to					thrombus	Process	growth of			NULL	at the sites of arterial injury	NULL	NULL	NULL	NULL	gw60_circulation_103_8_1128_s_141	11222477	36  The reactions of platelets are mostly integrin-dependent, involving the binding of platelet glycoprotein Ia/IIa to collagen and glycoprotein IIb/IIa to fibrinogen, which results in shape change, release of granule contents, and aggregation, leading to thrombus growth at the sites of arterial injury.	bind
32976	16	7942	5	13	NULL	NULL	NULL	statement 13	Process		leads to					thrombus	Process	growth of			NULL	at the sites of arterial injury	NULL	NULL	NULL	NULL	gw60_circulation_103_8_1128_s_141	11222477	36  The reactions of platelets are mostly integrin-dependent, involving the binding of platelet glycoprotein Ia/IIa to collagen and glycoprotein IIb/IIa to fibrinogen, which results in shape change, release of granule contents, and aggregation, leading to thrombus growth at the sites of arterial injury.	bind
25728	1	7942	6	NULL	NULL	0	NULL	platelet glycoprotein Ia/IIa	NULL		bind	NULL				collagen	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_8_1128_s_141	11222477	36  The reactions of platelets are mostly integrin-dependent, involving the binding of platelet glycoprotein Ia/IIa to collagen and glycoprotein IIb/IIa to fibrinogen, which results in shape change, release of granule contents, and aggregation, leading to thrombus growth at the sites of arterial injury.	bind
25729	2	7942	6	NULL	NULL	0	NULL	glycoprotein IIb/IIa	NULL		bind	NULL				fibrinogen	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_8_1128_s_141	11222477	36  The reactions of platelets are mostly integrin-dependent, involving the binding of platelet glycoprotein Ia/IIa to collagen and glycoprotein IIb/IIa to fibrinogen, which results in shape change, release of granule contents, and aggregation, leading to thrombus growth at the sites of arterial injury.	bind
25730	3	7942	6	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				integrin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_8_1128_s_141	11222477	36  The reactions of platelets are mostly integrin-dependent, involving the binding of platelet glycoprotein Ia/IIa to collagen and glycoprotein IIb/IIa to fibrinogen, which results in shape change, release of granule contents, and aggregation, leading to thrombus growth at the sites of arterial injury.	bind
25731	4	7942	6	NULL	NULL	0	NULL	statement 2	NULL		is dependent on	NULL				integrin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_8_1128_s_141	11222477	36  The reactions of platelets are mostly integrin-dependent, involving the binding of platelet glycoprotein Ia/IIa to collagen and glycoprotein IIb/IIa to fibrinogen, which results in shape change, release of granule contents, and aggregation, leading to thrombus growth at the sites of arterial injury.	bind
25732	5	7942	6	NULL	NULL	0	NULL	statement 1	NULL		results in	NULL				shape change	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_8_1128_s_141	11222477	36  The reactions of platelets are mostly integrin-dependent, involving the binding of platelet glycoprotein Ia/IIa to collagen and glycoprotein IIb/IIa to fibrinogen, which results in shape change, release of granule contents, and aggregation, leading to thrombus growth at the sites of arterial injury.	bind
25733	6	7942	6	NULL	NULL	0	NULL	statement 2	NULL		results in	NULL				shape change	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_8_1128_s_141	11222477	36  The reactions of platelets are mostly integrin-dependent, involving the binding of platelet glycoprotein Ia/IIa to collagen and glycoprotein IIb/IIa to fibrinogen, which results in shape change, release of granule contents, and aggregation, leading to thrombus growth at the sites of arterial injury.	bind
25734	7	7942	6	NULL	NULL	0	NULL	statement 1	NULL		results in	NULL				granule contents	NULL	release of			NULL		0	NULL	NULL	NULL	gw60_circulation_103_8_1128_s_141	11222477	36  The reactions of platelets are mostly integrin-dependent, involving the binding of platelet glycoprotein Ia/IIa to collagen and glycoprotein IIb/IIa to fibrinogen, which results in shape change, release of granule contents, and aggregation, leading to thrombus growth at the sites of arterial injury.	bind
25735	8	7942	6	NULL	NULL	0	NULL	statement 2	NULL		results in	NULL				granule contents	NULL	release of			NULL		0	NULL	NULL	NULL	gw60_circulation_103_8_1128_s_141	11222477	36  The reactions of platelets are mostly integrin-dependent, involving the binding of platelet glycoprotein Ia/IIa to collagen and glycoprotein IIb/IIa to fibrinogen, which results in shape change, release of granule contents, and aggregation, leading to thrombus growth at the sites of arterial injury.	bind
25736	9	7942	6	NULL	NULL	0	NULL	statement 1	NULL		results in	NULL				platelet aggregation	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_8_1128_s_141	11222477	36  The reactions of platelets are mostly integrin-dependent, involving the binding of platelet glycoprotein Ia/IIa to collagen and glycoprotein IIb/IIa to fibrinogen, which results in shape change, release of granule contents, and aggregation, leading to thrombus growth at the sites of arterial injury.	bind
25737	10	7942	6	NULL	NULL	0	NULL	statement 2	NULL		results in	NULL				platelet aggregation	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_8_1128_s_141	11222477	36  The reactions of platelets are mostly integrin-dependent, involving the binding of platelet glycoprotein Ia/IIa to collagen and glycoprotein IIb/IIa to fibrinogen, which results in shape change, release of granule contents, and aggregation, leading to thrombus growth at the sites of arterial injury.	bind
25738	11	7942	6	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				thrombus	NULL	growth of			NULL	sites of arterial injury	0	NULL	NULL	NULL	gw60_circulation_103_8_1128_s_141	11222477	36  The reactions of platelets are mostly integrin-dependent, involving the binding of platelet glycoprotein Ia/IIa to collagen and glycoprotein IIb/IIa to fibrinogen, which results in shape change, release of granule contents, and aggregation, leading to thrombus growth at the sites of arterial injury.	bind
25739	12	7942	6	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				thrombus	NULL	growth of			NULL	sites of arterial injury	0	NULL	NULL	NULL	gw60_circulation_103_8_1128_s_141	11222477	36  The reactions of platelets are mostly integrin-dependent, involving the binding of platelet glycoprotein Ia/IIa to collagen and glycoprotein IIb/IIa to fibrinogen, which results in shape change, release of granule contents, and aggregation, leading to thrombus growth at the sites of arterial injury.	bind
32977	1	7943	5	13	NULL	NULL	NULL	mAbs OB/04	GP		bind					oxLDL	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_5_704_s_144	7749884	36  We studied a possible cross-reactivity of the mAbs with acetylated LDL (REM, 3.3), comparing it with oxLDL (REM, 3.2; modified apoB, 40%) in preventing the binding of mAbs OB/04 and OB/09 to oxLDL in the wells at competitor concentrations from 0.01 mug/mL to 1 mg/mL.	bind
32978	2	7943	5	13	NULL	NULL	NULL	mAbs OB/09	GP		bind					oxLDL	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_5_704_s_144	7749884	36  We studied a possible cross-reactivity of the mAbs with acetylated LDL (REM, 3.3), comparing it with oxLDL (REM, 3.2; modified apoB, 40%) in preventing the binding of mAbs OB/04 and OB/09 to oxLDL in the wells at competitor concentrations from 0.01 mug/mL to 1 mg/mL.	bind
25514	1	7943	6	NULL	NULL	0	NULL	mAb OB/04	NULL		bind	NULL				OxLDL	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_5_704_s_144	7749884	36  We studied a possible cross-reactivity of the mAbs with acetylated LDL (REM, 3.3), comparing it with oxLDL (REM, 3.2; modified apoB, 40%) in preventing the binding of mAbs OB/04 and OB/09 to oxLDL in the wells at competitor concentrations from 0.01 mug/mL to 1 mg/mL.	bind
25515	2	7943	6	NULL	NULL	0	NULL	mAb OB/09	NULL		bind	NULL				oxLDL	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_5_704_s_144	7749884	36  We studied a possible cross-reactivity of the mAbs with acetylated LDL (REM, 3.3), comparing it with oxLDL (REM, 3.2; modified apoB, 40%) in preventing the binding of mAbs OB/04 and OB/09 to oxLDL in the wells at competitor concentrations from 0.01 mug/mL to 1 mg/mL.	bind
33048	1	7944	5	13	NULL	NULL	NULL	Sp1	GP		bind					LDL receptor gene	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_8_1248_s_214	7627719	36 37  Alternatively, we cannot rule out the possibility that cell cycle - specific cofactors are required for the enhancement of binding of Sp1 to the LDL receptor gene after PDGF stimulation.	bind
33049	2	7944	5	13	NULL	NULL	NULL	statement 1	Process		occurs after					PDGF	GP	stimulation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_8_1248_s_214	7627719	36 37  Alternatively, we cannot rule out the possibility that cell cycle - specific cofactors are required for the enhancement of binding of Sp1 to the LDL receptor gene after PDGF stimulation.	bind
33050	3	7944	5	13	NULL	NULL	NULL	cofactors	Chemical	cell cycle - specific 	is required for					statement 1	Process	enhancement of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_8_1248_s_214	7627719	36 37  Alternatively, we cannot rule out the possibility that cell cycle - specific cofactors are required for the enhancement of binding of Sp1 to the LDL receptor gene after PDGF stimulation.	bind
25524	2	7944	6	NULL	NULL	0	NULL	statement 1	NULL		occurs after	NULL				PDGF	NULL	stimulation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_8_1248_s_214	7627719	36 37  Alternatively, we cannot rule out the possibility that cell cycle - specific cofactors are required for the enhancement of binding of Sp1 to the LDL receptor gene after PDGF stimulation.	bind
25526	3	7944	6	NULL	NULL	0	NULL	cofactors	NULL	cell cycle specific	are required for	NULL				statement 1	NULL	enhancement of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_8_1248_s_214	7627719	36 37  Alternatively, we cannot rule out the possibility that cell cycle - specific cofactors are required for the enhancement of binding of Sp1 to the LDL receptor gene after PDGF stimulation.	bind
25535	1	7944	6	NULL	NULL	0	NULL	Sp1	NULL		bind	NULL				LDL receptor gene	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_8_1248_s_214	7627719	36 37  Alternatively, we cannot rule out the possibility that cell cycle - specific cofactors are required for the enhancement of binding of Sp1 to the LDL receptor gene after PDGF stimulation.	bind
33051	1	7945	5	13	NULL	NULL	NULL	LDL	GP		bind					collagen	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1375_s_134	7867176	36 37  In this respect, it is interesting that the binding of LDL to collagen may induce conformational changes in apo B that facilitate its binding to collagen-like domains of the scavenger receptor.	bind
33052	2	7945	5	13	NULL	NULL	NULL	statement 1	Process		induces		may			apo B	GP	conformational changes in			NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1375_s_134	7867176	36 37  In this respect, it is interesting that the binding of LDL to collagen may induce conformational changes in apo B that facilitate its binding to collagen-like domains of the scavenger receptor.	bind
33053	3	7945	5	13	NULL	NULL	NULL	apo B	GP		bind					scavenger receptor	GP		collagen-like domains		NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1375_s_134	7867176	36 37  In this respect, it is interesting that the binding of LDL to collagen may induce conformational changes in apo B that facilitate its binding to collagen-like domains of the scavenger receptor.	bind
36177	4	7945	5	13	NULL	NULL	NULL	statement 2	Process		facilitates					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1375_s_134	7867176	36 37  In this respect, it is interesting that the binding of LDL to collagen may induce conformational changes in apo B that facilitate its binding to collagen-like domains of the scavenger receptor.	bind
25536	1	7945	6	NULL	NULL	0	NULL	LDL	NULL		bind	NULL				collagen	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_91_5_1375_s_134	7867176	36 37  In this respect, it is interesting that the binding of LDL to collagen may induce conformational changes in apo B that facilitate its binding to collagen-like domains of the scavenger receptor.	bind
25537	2	7945	6	NULL	NULL	0	NULL	statement 1	NULL		induce	NULL	may			apo B	NULL	conformational change in			NULL		0	NULL	NULL	NULL	gw60_circulation_91_5_1375_s_134	7867176	36 37  In this respect, it is interesting that the binding of LDL to collagen may induce conformational changes in apo B that facilitate its binding to collagen-like domains of the scavenger receptor.	bind
25538	3	7945	6	NULL	NULL	0	NULL	apo B	NULL		bind	NULL				scavenger receptor	NULL		collagen-like domain		NULL		0	NULL	NULL	NULL	gw60_circulation_91_5_1375_s_134	7867176	36 37  In this respect, it is interesting that the binding of LDL to collagen may induce conformational changes in apo B that facilitate its binding to collagen-like domains of the scavenger receptor.	bind
25539	4	7945	6	NULL	NULL	0	NULL	statement 2	NULL		facilitates	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_91_5_1375_s_134	7867176	36 37  In this respect, it is interesting that the binding of LDL to collagen may induce conformational changes in apo B that facilitate its binding to collagen-like domains of the scavenger receptor.	bind
33054	1	7946	5	13	NULL	NULL	NULL	oligonucleotides	NucleicAcid		bind		potentially		four sequential guanosines	bFGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_3_669_s_176	9024156	36 37  It was hypothesized that oligonucleotides with four sequential guanosines might bind to serum proteins, including growth factors such as bFGF, acidic fibroblast growth factor, PDGF, and vascular endothelial growth factor, reducing the interaction of these growth factors with their receptors and the intracellular signal transduction leading to gene protein expression (such as c- myc and c- myb) involved in cell-cycle progression.	bind
33055	2	7946	5	13	NULL	NULL	NULL	bFGF	GP		is a type of					growth factors	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_3_669_s_176	9024156	36 37  It was hypothesized that oligonucleotides with four sequential guanosines might bind to serum proteins, including growth factors such as bFGF, acidic fibroblast growth factor, PDGF, and vascular endothelial growth factor, reducing the interaction of these growth factors with their receptors and the intracellular signal transduction leading to gene protein expression (such as c- myc and c- myb) involved in cell-cycle progression.	bind
33056	3	7946	5	13	NULL	NULL	NULL	bFGF	GP		is a type of					serum protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_3_669_s_176	9024156	36 37  It was hypothesized that oligonucleotides with four sequential guanosines might bind to serum proteins, including growth factors such as bFGF, acidic fibroblast growth factor, PDGF, and vascular endothelial growth factor, reducing the interaction of these growth factors with their receptors and the intracellular signal transduction leading to gene protein expression (such as c- myc and c- myb) involved in cell-cycle progression.	bind
33057	4	7946	5	13	NULL	NULL	NULL	oligonucleotides	NucleicAcid		bind		potentially		four sequential guanosines	PDGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_3_669_s_176	9024156	36 37  It was hypothesized that oligonucleotides with four sequential guanosines might bind to serum proteins, including growth factors such as bFGF, acidic fibroblast growth factor, PDGF, and vascular endothelial growth factor, reducing the interaction of these growth factors with their receptors and the intracellular signal transduction leading to gene protein expression (such as c- myc and c- myb) involved in cell-cycle progression.	bind
33058	5	7946	5	13	NULL	NULL	NULL	PDGF	GP		is a type of					acidic fibroblast growth factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_3_669_s_176	9024156	36 37  It was hypothesized that oligonucleotides with four sequential guanosines might bind to serum proteins, including growth factors such as bFGF, acidic fibroblast growth factor, PDGF, and vascular endothelial growth factor, reducing the interaction of these growth factors with their receptors and the intracellular signal transduction leading to gene protein expression (such as c- myc and c- myb) involved in cell-cycle progression.	bind
33059	6	7946	5	13	NULL	NULL	NULL	PDGF	GP		is a type of					serum protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_3_669_s_176	9024156	36 37  It was hypothesized that oligonucleotides with four sequential guanosines might bind to serum proteins, including growth factors such as bFGF, acidic fibroblast growth factor, PDGF, and vascular endothelial growth factor, reducing the interaction of these growth factors with their receptors and the intracellular signal transduction leading to gene protein expression (such as c- myc and c- myb) involved in cell-cycle progression.	bind
33060	7	7946	5	13	NULL	NULL	NULL	oligonucleotides	NucleicAcid		bind		potentially		four sequential guanosines	vascular endothelial growth factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_3_669_s_176	9024156	36 37  It was hypothesized that oligonucleotides with four sequential guanosines might bind to serum proteins, including growth factors such as bFGF, acidic fibroblast growth factor, PDGF, and vascular endothelial growth factor, reducing the interaction of these growth factors with their receptors and the intracellular signal transduction leading to gene protein expression (such as c- myc and c- myb) involved in cell-cycle progression.	bind
33061	8	7946	5	13	NULL	NULL	NULL	bFGF	GP		interacts with					receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_3_669_s_176	9024156	36 37  It was hypothesized that oligonucleotides with four sequential guanosines might bind to serum proteins, including growth factors such as bFGF, acidic fibroblast growth factor, PDGF, and vascular endothelial growth factor, reducing the interaction of these growth factors with their receptors and the intracellular signal transduction leading to gene protein expression (such as c- myc and c- myb) involved in cell-cycle progression.	bind
33062	9	7946	5	13	NULL	NULL	NULL	statement 1	Process		reduces					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_3_669_s_176	9024156	36 37  It was hypothesized that oligonucleotides with four sequential guanosines might bind to serum proteins, including growth factors such as bFGF, acidic fibroblast growth factor, PDGF, and vascular endothelial growth factor, reducing the interaction of these growth factors with their receptors and the intracellular signal transduction leading to gene protein expression (such as c- myc and c- myb) involved in cell-cycle progression.	bind
33063	10	7946	5	13	NULL	NULL	NULL	PDGF	GP		interacts with					receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_3_669_s_176	9024156	36 37  It was hypothesized that oligonucleotides with four sequential guanosines might bind to serum proteins, including growth factors such as bFGF, acidic fibroblast growth factor, PDGF, and vascular endothelial growth factor, reducing the interaction of these growth factors with their receptors and the intracellular signal transduction leading to gene protein expression (such as c- myc and c- myb) involved in cell-cycle progression.	bind
33064	11	7946	5	13	NULL	NULL	NULL	statement 4	Process		reduces					statement 10	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_3_669_s_176	9024156	36 37  It was hypothesized that oligonucleotides with four sequential guanosines might bind to serum proteins, including growth factors such as bFGF, acidic fibroblast growth factor, PDGF, and vascular endothelial growth factor, reducing the interaction of these growth factors with their receptors and the intracellular signal transduction leading to gene protein expression (such as c- myc and c- myb) involved in cell-cycle progression.	bind
33065	12	7946	5	13	NULL	NULL	NULL	vascular endothelial growth factor	GP		interacts with					receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_3_669_s_176	9024156	36 37  It was hypothesized that oligonucleotides with four sequential guanosines might bind to serum proteins, including growth factors such as bFGF, acidic fibroblast growth factor, PDGF, and vascular endothelial growth factor, reducing the interaction of these growth factors with their receptors and the intracellular signal transduction leading to gene protein expression (such as c- myc and c- myb) involved in cell-cycle progression.	bind
33066	13	7946	5	13	NULL	NULL	NULL	statement 7	Process		reduces					statement 12	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_3_669_s_176	9024156	36 37  It was hypothesized that oligonucleotides with four sequential guanosines might bind to serum proteins, including growth factors such as bFGF, acidic fibroblast growth factor, PDGF, and vascular endothelial growth factor, reducing the interaction of these growth factors with their receptors and the intracellular signal transduction leading to gene protein expression (such as c- myc and c- myb) involved in cell-cycle progression.	bind
33069	14	7946	5	13	NULL	NULL	NULL	c- myc	GP		is involved in					cell-cycle 	Process	progression of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_3_669_s_176	9024156	36 37  It was hypothesized that oligonucleotides with four sequential guanosines might bind to serum proteins, including growth factors such as bFGF, acidic fibroblast growth factor, PDGF, and vascular endothelial growth factor, reducing the interaction of these growth factors with their receptors and the intracellular signal transduction leading to gene protein expression (such as c- myc and c- myb) involved in cell-cycle progression.	bind
33070	15	7946	5	13	NULL	NULL	NULL	c- myb	GP		is involved in					cell-cycle	Process	progression of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_3_669_s_176	9024156	36 37  It was hypothesized that oligonucleotides with four sequential guanosines might bind to serum proteins, including growth factors such as bFGF, acidic fibroblast growth factor, PDGF, and vascular endothelial growth factor, reducing the interaction of these growth factors with their receptors and the intracellular signal transduction leading to gene protein expression (such as c- myc and c- myb) involved in cell-cycle progression.	bind
25723	1	7946	6	NULL	NULL	0	NULL	oligonucleotides with four sequential guanosines	NULL		bind	NULL	may			bFGF	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_95_3_669_s_176	9024156	36 37  It was hypothesized that oligonucleotides with four sequential guanosines might bind to serum proteins, including growth factors such as bFGF, acidic fibroblast growth factor, PDGF, and vascular endothelial growth factor, reducing the interaction of these growth factors with their receptors and the intracellular signal transduction leading to gene protein expression (such as c- myc and c- myb) involved in cell-cycle progression.	bind
25724	2	7946	6	NULL	NULL	0	NULL	oligonucleotides with four sequential guanosines	NULL		bind	NULL	may			acidic fibroblast growth factor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_95_3_669_s_176	9024156	36 37  It was hypothesized that oligonucleotides with four sequential guanosines might bind to serum proteins, including growth factors such as bFGF, acidic fibroblast growth factor, PDGF, and vascular endothelial growth factor, reducing the interaction of these growth factors with their receptors and the intracellular signal transduction leading to gene protein expression (such as c- myc and c- myb) involved in cell-cycle progression.	bind
25725	3	7946	6	NULL	NULL	0	NULL	oligonucleotides with four sequential guanosines	NULL		bind	NULL	may			vascular endothelial growth factor	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_3_669_s_176	9024156	36 37  It was hypothesized that oligonucleotides with four sequential guanosines might bind to serum proteins, including growth factors such as bFGF, acidic fibroblast growth factor, PDGF, and vascular endothelial growth factor, reducing the interaction of these growth factors with their receptors and the intracellular signal transduction leading to gene protein expression (such as c- myc and c- myb) involved in cell-cycle progression.	bind
25726	4	7946	6	NULL	NULL	0	NULL	oligonucleotides with four sequential guanosines	NULL		bind	NULL	may			PDGF	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_3_669_s_176	9024156	36 37  It was hypothesized that oligonucleotides with four sequential guanosines might bind to serum proteins, including growth factors such as bFGF, acidic fibroblast growth factor, PDGF, and vascular endothelial growth factor, reducing the interaction of these growth factors with their receptors and the intracellular signal transduction leading to gene protein expression (such as c- myc and c- myb) involved in cell-cycle progression.	bind
25727	5	7946	6	NULL	NULL	0	NULL	bFGF	NULL		is a type of	NULL				growth factor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_95_3_669_s_176	9024156	36 37  It was hypothesized that oligonucleotides with four sequential guanosines might bind to serum proteins, including growth factors such as bFGF, acidic fibroblast growth factor, PDGF, and vascular endothelial growth factor, reducing the interaction of these growth factors with their receptors and the intracellular signal transduction leading to gene protein expression (such as c- myc and c- myb) involved in cell-cycle progression.	bind
26089	6	7946	6	NULL	NULL	0	NULL	PDGF	NULL		is a type of	NULL				growth factor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_95_3_669_s_176	9024156	36 37  It was hypothesized that oligonucleotides with four sequential guanosines might bind to serum proteins, including growth factors such as bFGF, acidic fibroblast growth factor, PDGF, and vascular endothelial growth factor, reducing the interaction of these growth factors with their receptors and the intracellular signal transduction leading to gene protein expression (such as c- myc and c- myb) involved in cell-cycle progression.	bind
33898	1	7947	5	13	NULL	NULL	NULL	apoE	GP		bind					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_149_s_244	9012650	36 37  Thus, eliminating only one of the positive charges in the LDL receptor - binding segment of apoE may reduce the affinity of apoE (dimer) in VLDL or a liposome to the level of affinity of apoB-100 in LDL for the LDL receptor.	bind
33902	3	7947	5	13	NULL	NULL	NULL	statement 2	Process		reduce		may			apoE (dimer)	GP	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_149_s_244	9012650	36 37  Thus, eliminating only one of the positive charges in the LDL receptor - binding segment of apoE may reduce the affinity of apoE (dimer) in VLDL or a liposome to the level of affinity of apoB-100 in LDL for the LDL receptor.	bind
33904	4	7947	5	13	NULL	NULL	NULL	apoB-100	GP		bind					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_149_s_244	9012650	36 37  Thus, eliminating only one of the positive charges in the LDL receptor - binding segment of apoE may reduce the affinity of apoE (dimer) in VLDL or a liposome to the level of affinity of apoB-100 in LDL for the LDL receptor.	bind
36176	2	7947	5	13	NULL	NULL	NULL	one positive charge	Chemical		is eliminated from					apoE	GP		LDL receptor - binding segment		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_149_s_244	9012650	36 37  Thus, eliminating only one of the positive charges in the LDL receptor - binding segment of apoE may reduce the affinity of apoE (dimer) in VLDL or a liposome to the level of affinity of apoB-100 in LDL for the LDL receptor.	bind
25718	1	7947	6	NULL	NULL	0	NULL	apoE (dimer)	NULL		bind	NULL				VLDL	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_149_s_244	9012650	36 37  Thus, eliminating only one of the positive charges in the LDL receptor - binding segment of apoE may reduce the affinity of apoE (dimer) in VLDL or a liposome to the level of affinity of apoB-100 in LDL for the LDL receptor.	bind
25722	2	7947	6	NULL	NULL	0	NULL	apoE	NULL	elimination of	reduces	NULL		LDL receptor - binding segment		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_149_s_244	9012650	36 37  Thus, eliminating only one of the positive charges in the LDL receptor - binding segment of apoE may reduce the affinity of apoE (dimer) in VLDL or a liposome to the level of affinity of apoB-100 in LDL for the LDL receptor.	bind
33077	1	7948	5	13	NULL	NULL	NULL	ROS	Chemical		is generated during					strain					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_7_804_s_44	10205148	36 37 38 39  We also illustrated that strain-induced MCP-1 expression was a result of increased activator protein-1 binding by ROS generated during strain.	bind
33078	2	7948	5	13	NULL	NULL	NULL	statement 1	Chemical		bind					activator protein-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_7_804_s_44	10205148	36 37 38 39  We also illustrated that strain-induced MCP-1 expression was a result of increased activator protein-1 binding by ROS generated during strain.	bind
33079	4	7948	5	13	NULL	NULL	NULL	statement 2	Process	increase in	results in					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_7_804_s_44	10205148	36 37 38 39  We also illustrated that strain-induced MCP-1 expression was a result of increased activator protein-1 binding by ROS generated during strain.	bind
33080	3	7948	5	13	NULL	NULL	NULL	strain			induces					MCP-1	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_7_804_s_44	10205148	36 37 38 39  We also illustrated that strain-induced MCP-1 expression was a result of increased activator protein-1 binding by ROS generated during strain.	bind
25540	1	7948	6	NULL	NULL	0	NULL	strain	NULL		induces	NULL				MCP-1	NULL	expression of			NULL		0	NULL	NULL	NULL	gw60_circulationres_84_7_804_s_44	10205148	36 37 38 39  We also illustrated that strain-induced MCP-1 expression was a result of increased activator protein-1 binding by ROS generated during strain.	bind
25542	2	7948	6	NULL	NULL	0	NULL	activator protein-1 	NULL		bind	NULL				ROS	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_7_804_s_44	10205148	36 37 38 39  We also illustrated that strain-induced MCP-1 expression was a result of increased activator protein-1 binding by ROS generated during strain.	bind
25544	3	7948	6	NULL	NULL	0	NULL	ROS	NULL		is generated during	NULL				strain	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_7_804_s_44	10205148	36 37 38 39  We also illustrated that strain-induced MCP-1 expression was a result of increased activator protein-1 binding by ROS generated during strain.	bind
37313	4	7948	6	NULL	NULL	0	NULL	statement 2	NULL		occurs by	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_7_804_s_44	10205148	36 37 38 39  We also illustrated that strain-induced MCP-1 expression was a result of increased activator protein-1 binding by ROS generated during strain.	bind
33081	1	7949	5	13	NULL	NULL	NULL	importin	GP		bind								NLS		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_35_22134_s_123	9268357	36 and  42), that the initial events of nuclear transport, and NLS-binding by importin in particular, are critical in determining overall nuclear protein import kinetics.	bind
33082	2	7949	5	13	NULL	NULL	NULL	statement 1	Process		determines					nuclear protein import kinetics	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_35_22134_s_123	9268357	36 and  42), that the initial events of nuclear transport, and NLS-binding by importin in particular, are critical in determining overall nuclear protein import kinetics.	bind
33083	3	7949	5	13	NULL	NULL	NULL	statement 1	Process		is initial event of					nuclear transport	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_35_22134_s_123	9268357	36 and  42), that the initial events of nuclear transport, and NLS-binding by importin in particular, are critical in determining overall nuclear protein import kinetics.	bind
25545	1	7949	6	NULL	NULL	0	NULL	NLS	NULL		bind	NULL				importin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_35_22134_s_123	9268357	36 and  42), that the initial events of nuclear transport, and NLS-binding by importin in particular, are critical in determining overall nuclear protein import kinetics.	bind
33151	1	7950	5	13	NULL	NULL	NULL	36 peptide antibody	GP		is directed to					alpha3(IV)NC1	GP		last 36 residues containing COOH-terminal epitope		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_26_20027_s_100	10748075	36 peptide antibody directed to the last 36 residues containing the COOH-terminal epitope in the alpha3(IV)NC1 bound equally well to the NC1 hexamer and the control antibody, demonstrating that all epitopes were now exposed for binding.	bind
33162	2	7950	5	13	NULL	NULL	NULL	36 peptide antibody	GP		bind					NC1 hexamer	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_26_20027_s_100	10748075	36 peptide antibody directed to the last 36 residues containing the COOH-terminal epitope in the alpha3(IV)NC1 bound equally well to the NC1 hexamer and the control antibody, demonstrating that all epitopes were now exposed for binding.	bind
25695	2	7950	6	10	NULL	0	NULL	36 peptide antibody			bind					NC1 hexamer					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_26_20027_s_100	10748075	36 peptide antibody directed to the last 36 residues containing the COOH-terminal epitope in the alpha3(IV)NC1 bound equally well to the NC1 hexamer and the control antibody, demonstrating that all epitopes were now exposed for binding.	bind
25700	1	7950	6	10	NULL	0	NULL	36 peptide antibody			is directed to					alpha3(IV)NC1			last 36 residues containing COOH-terminal epitope		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_26_20027_s_100	10748075	36 peptide antibody directed to the last 36 residues containing the COOH-terminal epitope in the alpha3(IV)NC1 bound equally well to the NC1 hexamer and the control antibody, demonstrating that all epitopes were now exposed for binding.	bind
33084	1	7951	5	13	NULL	NULL	NULL	thrombin	GP		stimulates					VCAM-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_41_s_118	14551154	36 Similarly, thrombin stimulation of VCAM-1 involves the inducible binding of p65 NF-kappaB to a tandem NF-kappaB motif in the 5' flanking region.	bind
33085	2	7951	5	13	NULL	NULL	NULL	p65 NF-kappaB	GP		bind									tandem NF-kappaB motif in 5' flanking region	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_41_s_118	14551154	36 Similarly, thrombin stimulation of VCAM-1 involves the inducible binding of p65 NF-kappaB to a tandem NF-kappaB motif in the 5' flanking region.	bind
33086	3	7951	5	13	NULL	NULL	NULL	statement 1	Process		involves					statement 2	Process	inducible			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_41_s_118	14551154	36 Similarly, thrombin stimulation of VCAM-1 involves the inducible binding of p65 NF-kappaB to a tandem NF-kappaB motif in the 5' flanking region.	bind
25546	1	7951	6	NULL	NULL	0	NULL	p65 NF-kappaB	NULL		bind	NULL					NULL			tandem NF-kappaB motif in 5' flanking region	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_41_s_118	14551154	36 Similarly, thrombin stimulation of VCAM-1 involves the inducible binding of p65 NF-kappaB to a tandem NF-kappaB motif in the 5' flanking region.	bind
25547	2	7951	6	NULL	NULL	0	NULL	thrombin	NULL		stimulates	NULL				VCAM-1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_41_s_118	14551154	36 Similarly, thrombin stimulation of VCAM-1 involves the inducible binding of p65 NF-kappaB to a tandem NF-kappaB motif in the 5' flanking region.	bind
25548	3	7951	6	NULL	NULL	0	NULL	statement 2	NULL		induces	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_41_s_118	14551154	36 Similarly, thrombin stimulation of VCAM-1 involves the inducible binding of p65 NF-kappaB to a tandem NF-kappaB motif in the 5' flanking region.	bind
33169	1	7952	5	13	NULL	NULL	NULL	nuclear proteins	GP		bind									Egr-1 consensus DNA sequence	NULL	mouse macrophages	NULL	NULL	NULL	NULL	gw70_circulationres_94_3_333_s_170	14670837	36 When these concepts were probed in tissue culture, these investigators found that mouse macrophages displayed decreased lipopolysaccharide-induced binding of nuclear proteins to the Egr-1 consensus DNA sequence after pretreatment with simvastatin.	bind
33172	2	7952	5	13	NULL	NULL	NULL	lipopolysaccharide	Chemical		induces					statement 1	Process				NULL	mouse macrophages	NULL	NULL	NULL	NULL	gw70_circulationres_94_3_333_s_170	14670837	36 When these concepts were probed in tissue culture, these investigators found that mouse macrophages displayed decreased lipopolysaccharide-induced binding of nuclear proteins to the Egr-1 consensus DNA sequence after pretreatment with simvastatin.	bind
33174	3	7952	5	13	NULL	NULL	NULL	simvastatin	Chemical	pretreatment	decrease					statement 2	Process				NULL	mouse macrophages	NULL	NULL	NULL	NULL	gw70_circulationres_94_3_333_s_170	14670837	36 When these concepts were probed in tissue culture, these investigators found that mouse macrophages displayed decreased lipopolysaccharide-induced binding of nuclear proteins to the Egr-1 consensus DNA sequence after pretreatment with simvastatin.	bind
25549	1	7952	6	NULL	NULL	0	NULL	nuclear proteins	NULL		bind	NULL					NULL			Egr-1 consensus DNA sequence	NULL	mouse macrophages	NULL	NULL	NULL	NULL	gw70_circulationres_94_3_333_s_170	14670837	36 When these concepts were probed in tissue culture, these investigators found that mouse macrophages displayed decreased lipopolysaccharide-induced binding of nuclear proteins to the Egr-1 consensus DNA sequence after pretreatment with simvastatin.	bind
25550	2	7952	6	NULL	NULL	0	NULL	lipopolysaccharide	NULL		induces	NULL				statement 1	NULL				NULL	mouse macrophages	NULL	NULL	NULL	NULL	gw70_circulationres_94_3_333_s_170	14670837	36 When these concepts were probed in tissue culture, these investigators found that mouse macrophages displayed decreased lipopolysaccharide-induced binding of nuclear proteins to the Egr-1 consensus DNA sequence after pretreatment with simvastatin.	bind
25552	3	7952	6	NULL	NULL	0	NULL	simvastatin	NULL	pretreatment with	decreases	NULL				statement 2	NULL				NULL	mouse macrophages	NULL	NULL	NULL	NULL	gw70_circulationres_94_3_333_s_170	14670837	36 When these concepts were probed in tissue culture, these investigators found that mouse macrophages displayed decreased lipopolysaccharide-induced binding of nuclear proteins to the Egr-1 consensus DNA sequence after pretreatment with simvastatin.	bind
33175	1	7953	5	13	NULL	NULL	NULL	p47 phox	GP		bind			N-terminal SH3 domain		p22 phox	GP		proline-rich region		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_4_453_s_63	16514078	36,41,42   The p47 phox N-terminal SH3 domain then binds the proline-rich region in p22 phox 42,43  and the PX domain of p47 phox binds 3'phosphoinositides, the products of PI3K.	bind
33179	2	7953	5	13	NULL	NULL	NULL	p47 phox	GP		bind			PX domain		3'phosphoinositides	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_4_453_s_63	16514078	36,41,42   The p47 phox N-terminal SH3 domain then binds the proline-rich region in p22 phox 42,43  and the PX domain of p47 phox binds 3'phosphoinositides, the products of PI3K.	bind
33181	3	7953	5	13	NULL	NULL	NULL	3'phosphoinositides	Chemical		is a product of					PI3K	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_4_453_s_63	16514078	36,41,42   The p47 phox N-terminal SH3 domain then binds the proline-rich region in p22 phox 42,43  and the PX domain of p47 phox binds 3'phosphoinositides, the products of PI3K.	bind
25553	1	7953	6	NULL	NULL	0	NULL	p47 phox	NULL		bind	NULL		N-terminal SH3 domain		p22 phox	NULL		proline-rich region		NULL		0	NULL	NULL	NULL	gw70_circulationres_98_4_453_s_63	16514078	36,41,42   The p47 phox N-terminal SH3 domain then binds the proline-rich region in p22 phox 42,43  and the PX domain of p47 phox binds 3'phosphoinositides, the products of PI3K.	bind
25554	2	7953	6	NULL	NULL	0	NULL	p47 phox	NULL		bind	NULL		PX domain		3' phosphoinositides	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_4_453_s_63	16514078	36,41,42   The p47 phox N-terminal SH3 domain then binds the proline-rich region in p22 phox 42,43  and the PX domain of p47 phox binds 3'phosphoinositides, the products of PI3K.	bind
25555	3	7953	6	NULL	NULL	0	NULL	3' phosphoinositides	NULL		are products of	NULL				PI3K	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_4_453_s_63	16514078	36,41,42   The p47 phox N-terminal SH3 domain then binds the proline-rich region in p22 phox 42,43  and the PX domain of p47 phox binds 3'phosphoinositides, the products of PI3K.	bind
33188	1	7954	5	13	NULL	NULL	NULL	unidentified protein	GP		bind							mice		Sp1 sites	NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_1129_s_166	11549606	36- [[ 38  This latter defect ]] is exemplified by the adenine phosphoribosyltransferase gene in mice, in which an unidentified protein that binds to the Sp1 sites seems to prevent methylation of the CpG island.	bind
33190	2	7954	5	13	NULL	NULL	NULL	statement 1	Process		prevents		may					methylation of		CpG island	NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_1129_s_166	11549606	36- [[ 38  This latter defect ]] is exemplified by the adenine phosphoribosyltransferase gene in mice, in which an unidentified protein that binds to the Sp1 sites seems to prevent methylation of the CpG island.	bind
25556	1	7954	6	NULL	NULL	0	NULL	unidentified protein	NULL		bind	NULL					NULL			Sp1 site	NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_3_1129_s_166	11549606	36- [[ 38  This latter defect ]] is exemplified by the adenine phosphoribosyltransferase gene in mice, in which an unidentified protein that binds to the Sp1 sites seems to prevent methylation of the CpG island.	bind
25557	2	7954	6	NULL	NULL	0	NULL	statement 1	NULL		prevent	NULL	may				NULL	methylation of 		CpG island	NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_1129_s_166	11549606	36- [[ 38  This latter defect ]] is exemplified by the adenine phosphoribosyltransferase gene in mice, in which an unidentified protein that binds to the Sp1 sites seems to prevent methylation of the CpG island.	bind
33191	1	7955	5	13	NULL	NULL	NULL	VLDL particle	GP		bind					CLA-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2341_s_169	9409200	37  According to this model, the large size of a given VLDL particle bound to CLA-1 may impede, by steric hindrance, the binding of other VLDL particles to nearby unoccupied receptors but not the binding of the much smaller particles such as HDL.	bind
33813	2	7955	5	13	NULL	NULL	NULL	VLDL particles	GP		bind					unoccupied receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2341_s_169	9409200	37  According to this model, the large size of a given VLDL particle bound to CLA-1 may impede, by steric hindrance, the binding of other VLDL particles to nearby unoccupied receptors but not the binding of the much smaller particles such as HDL.	bind
33815	4	7955	5	13	NULL	NULL	NULL	statement 1	Process		impede		may			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2341_s_169	9409200	37  According to this model, the large size of a given VLDL particle bound to CLA-1 may impede, by steric hindrance, the binding of other VLDL particles to nearby unoccupied receptors but not the binding of the much smaller particles such as HDL.	bind
33816	5	7955	5	13	NULL	NULL	NULL	statement 4	Process		occurs by					steric hindrance	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2341_s_169	9409200	37  According to this model, the large size of a given VLDL particle bound to CLA-1 may impede, by steric hindrance, the binding of other VLDL particles to nearby unoccupied receptors but not the binding of the much smaller particles such as HDL.	bind
33817	6	7955	5	13	NULL	NULL	NULL	statement 1	Process		does not impede					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2341_s_169	9409200	37  According to this model, the large size of a given VLDL particle bound to CLA-1 may impede, by steric hindrance, the binding of other VLDL particles to nearby unoccupied receptors but not the binding of the much smaller particles such as HDL.	bind
25558	1	7955	6	NULL	NULL	0	NULL	VLDL particle	NULL	large size of	bind	NULL				CLA-1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2341_s_169	9409200	37  According to this model, the large size of a given VLDL particle bound to CLA-1 may impede, by steric hindrance, the binding of other VLDL particles to nearby unoccupied receptors but not the binding of the much smaller particles such as HDL.	bind
25559	2	7955	6	NULL	NULL	0	NULL	VLDL particle	NULL		bind	NULL				unoccupied receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2341_s_169	9409200	37  According to this model, the large size of a given VLDL particle bound to CLA-1 may impede, by steric hindrance, the binding of other VLDL particles to nearby unoccupied receptors but not the binding of the much smaller particles such as HDL.	bind
25560	3	7955	6	NULL	NULL	0	NULL	statement 1	NULL		impede	NULL	may			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2341_s_169	9409200	37  According to this model, the large size of a given VLDL particle bound to CLA-1 may impede, by steric hindrance, the binding of other VLDL particles to nearby unoccupied receptors but not the binding of the much smaller particles such as HDL.	bind
25561	4	7955	6	NULL	NULL	0	NULL	HDL	NULL		bind	NULL				receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2341_s_169	9409200	37  According to this model, the large size of a given VLDL particle bound to CLA-1 may impede, by steric hindrance, the binding of other VLDL particles to nearby unoccupied receptors but not the binding of the much smaller particles such as HDL.	bind
25562	5	7955	6	NULL	NULL	0	NULL	statement 1	NULL		does not impede	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2341_s_169	9409200	37  According to this model, the large size of a given VLDL particle bound to CLA-1 may impede, by steric hindrance, the binding of other VLDL particles to nearby unoccupied receptors but not the binding of the much smaller particles such as HDL.	bind
33200	1	7956	5	13	NULL	NULL	NULL	laminin	GP		bind					apo(a)	GP	recombinant			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_5_1162_s_177	10323765	37  Also laminin and fibrinogen bind recombinant apo(a).	bind
33202	2	7956	5	13	NULL	NULL	NULL	fibrinogen	GP		bind					apo(a)	GP	recombinant			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_5_1162_s_177	10323765	37  Also laminin and fibrinogen bind recombinant apo(a).	bind
25563	1	7956	6	NULL	NULL	0	NULL	laminin	NULL		bind	NULL				apo(a)	NULL	recombinant			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_5_1162_s_177	10323765	37  Also laminin and fibrinogen bind recombinant apo(a).	bind
25564	2	7956	6	NULL	NULL	0	NULL	fibrinogen	NULL		bind	NULL				apo(a)	NULL	recombinant			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_5_1162_s_177	10323765	37  Also laminin and fibrinogen bind recombinant apo(a).	bind
33204	1	7957	5	13	NULL	NULL	NULL	c-Jun homodimers	GP		bind									TRE at -58 to -50	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3025_s_208	10591684	37  Binding of c-Jun homodimers to TRE at positions -58 to -50 is important in the basal activity and phorbol 12-myristate 13-acetate activation of the PAI-1 promoter in HepG2 cells.	bind
33206	2	7957	5	13	NULL	NULL	NULL	statement 1	Process		is important in					basal activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3025_s_208	10591684	37  Binding of c-Jun homodimers to TRE at positions -58 to -50 is important in the basal activity and phorbol 12-myristate 13-acetate activation of the PAI-1 promoter in HepG2 cells.	bind
33207	3	7957	5	13	NULL	NULL	NULL	phorbol 12-myristate 13-acetate	Chemical		activates					PAI-1	GP			promoter	NULL	in HepG2 cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3025_s_208	10591684	37  Binding of c-Jun homodimers to TRE at positions -58 to -50 is important in the basal activity and phorbol 12-myristate 13-acetate activation of the PAI-1 promoter in HepG2 cells.	bind
33208	4	7957	5	13	NULL	NULL	NULL	statement 1	Process		is important in					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3025_s_208	10591684	37  Binding of c-Jun homodimers to TRE at positions -58 to -50 is important in the basal activity and phorbol 12-myristate 13-acetate activation of the PAI-1 promoter in HepG2 cells.	bind
25565	1	7957	6	NULL	NULL	0	NULL		NULL		is located at	NULL			TRE		NULL			-58 to -50	NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3025_s_208	10591684	37  Binding of c-Jun homodimers to TRE at positions -58 to -50 is important in the basal activity and phorbol 12-myristate 13-acetate activation of the PAI-1 promoter in HepG2 cells.	bind
25566	2	7957	6	NULL	NULL	0	NULL	c-jun homodimers	NULL		bind	NULL					NULL			TRE	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3025_s_208	10591684	37  Binding of c-Jun homodimers to TRE at positions -58 to -50 is important in the basal activity and phorbol 12-myristate 13-acetate activation of the PAI-1 promoter in HepG2 cells.	bind
25567	3	7957	6	NULL	NULL	0	NULL	statement 2	NULL		is important for	NULL				basal activity	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3025_s_208	10591684	37  Binding of c-Jun homodimers to TRE at positions -58 to -50 is important in the basal activity and phorbol 12-myristate 13-acetate activation of the PAI-1 promoter in HepG2 cells.	bind
25568	4	7957	6	NULL	NULL	0	NULL	phorbol 12-myristate 13-acetate	NULL		activates	NULL				PAI-1	NULL			promoter	NULL	HepG2 cells	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3025_s_208	10591684	37  Binding of c-Jun homodimers to TRE at positions -58 to -50 is important in the basal activity and phorbol 12-myristate 13-acetate activation of the PAI-1 promoter in HepG2 cells.	bind
25569	5	7957	6	NULL	NULL	0	NULL	statement 2	NULL		is important for	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3025_s_208	10591684	37  Binding of c-Jun homodimers to TRE at positions -58 to -50 is important in the basal activity and phorbol 12-myristate 13-acetate activation of the PAI-1 promoter in HepG2 cells.	bind
33210	3	7958	5	13	NULL	NULL	NULL	statement 2	Process		attenuates					ischemia reperfusion injury	MedicalFinding				NULL	in myocardium	NULL	NULL	NULL	NULL	gw60_circulationres_86_2_139_s_127	10666408	37  In addition, it has recently been reported that transfecting rat hearts with a  cis element decoy against NF-kappaB binding site attenuates ischemia reperfusion injury in the myocardium.	bind
47831	1	7958	5	10	NULL	0	NULL		NULL		target against	NULL			cis element decoy		NULL			NF-kappaB binding site 	NULL		0	NULL	NULL	NULL	gw60_circulationres_86_2_139_s_127	10666408	37  In addition, it has recently been reported that transfecting rat hearts with a  cis element decoy against NF-kappaB binding site attenuates ischemia reperfusion injury in the myocardium.	bind
47832	2	7958	5	13	NULL	NULL	NULL	heart	OrganismPart	rat	transfected with					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_2_139_s_127	10666408	37  In addition, it has recently been reported that transfecting rat hearts with a  cis element decoy against NF-kappaB binding site attenuates ischemia reperfusion injury in the myocardium.	bind
25687	1	7958	6	NULL	NULL	0	NULL		NULL		targets against	NULL			cis element decoy		NULL			NF-kappaB binding site	NULL		0	NULL	NULL	NULL	gw60_circulationres_86_2_139_s_127	10666408	37  In addition, it has recently been reported that transfecting rat hearts with a  cis element decoy against NF-kappaB binding site attenuates ischemia reperfusion injury in the myocardium.	bind
25689	2	7958	6	10	NULL	0	NULL	 heart	NULL	rat	transfected with	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_2_139_s_127	10666408	37  In addition, it has recently been reported that transfecting rat hearts with a  cis element decoy against NF-kappaB binding site attenuates ischemia reperfusion injury in the myocardium.	bind
25690	3	7958	6	NULL	NULL	0	NULL	statement 2	NULL		attenuates	NULL				ischemia reperfusion injury	NULL				NULL	myocardium	0	NULL	NULL	NULL	gw60_circulationres_86_2_139_s_127	10666408	37  In addition, it has recently been reported that transfecting rat hearts with a  cis element decoy against NF-kappaB binding site attenuates ischemia reperfusion injury in the myocardium.	bind
33211	1	7959	5	13	NULL	NULL	NULL	C4	GP		bind		aspecific			myocardium	OrganismPart	infarcted			NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_1_97_s_149	8994423	37  Therefore, positive immunostaining with these MAbs ruled out the possibility that the results were influenced by aspecific binding of C4 and C3 to the infarcted myocardium.	bind
33212	2	7959	5	13	NULL	NULL	NULL	C3	GP		bind		aspecific			myocardium	OrganismPart	infarcted			NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_1_97_s_149	8994423	37  Therefore, positive immunostaining with these MAbs ruled out the possibility that the results were influenced by aspecific binding of C4 and C3 to the infarcted myocardium.	bind
25570	1	7959	6	NULL	NULL	0	NULL	C4	NULL		bind	NULL	aspecifically			myocardium	NULL	infarcted			NULL		0	NULL	NULL	NULL	gw60_circulation_95_1_97_s_149	8994423	37  Therefore, positive immunostaining with these MAbs ruled out the possibility that the results were influenced by aspecific binding of C4 and C3 to the infarcted myocardium.	bind
25571	2	7959	6	NULL	NULL	0	NULL	C3	NULL		bind	NULL	aspecifically			myocardium	NULL	infarcted			NULL		0	NULL	NULL	NULL	gw60_circulation_95_1_97_s_149	8994423	37  Therefore, positive immunostaining with these MAbs ruled out the possibility that the results were influenced by aspecific binding of C4 and C3 to the infarcted myocardium.	bind
33221	1	7960	5	13	NULL	NULL	NULL	p27Kip1	GP		bind					cyclin D/CDK4 complexes	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_3_1091_s_239	11238057	37  These changes will disrupt binding of p27Kip1 to cyclin D/CDK4 complexes leading to a redistribution and binding of p27Kip1 to cyclin E/CDK2 and cyclin A/CDK2 complexes with their inhibition.	bind
33223	2	7960	5	13	NULL	NULL	NULL	p27Kip1	GP		bind					cyclin E/cdk2 complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_3_1091_s_239	11238057	37  These changes will disrupt binding of p27Kip1 to cyclin D/CDK4 complexes leading to a redistribution and binding of p27Kip1 to cyclin E/CDK2 and cyclin A/CDK2 complexes with their inhibition.	bind
33224	3	7960	5	13	NULL	NULL	NULL	p27Kip1	GP		bind					cyclin A/CDK2 complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_3_1091_s_239	11238057	37  These changes will disrupt binding of p27Kip1 to cyclin D/CDK4 complexes leading to a redistribution and binding of p27Kip1 to cyclin E/CDK2 and cyclin A/CDK2 complexes with their inhibition.	bind
33226	4	7960	5	13	NULL	NULL	NULL	statement 1	Process	disruption of	leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_3_1091_s_239	11238057	37  These changes will disrupt binding of p27Kip1 to cyclin D/CDK4 complexes leading to a redistribution and binding of p27Kip1 to cyclin E/CDK2 and cyclin A/CDK2 complexes with their inhibition.	bind
33227	5	7960	5	13	NULL	NULL	NULL	statement 1	Process	disruption of	leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_3_1091_s_239	11238057	37  These changes will disrupt binding of p27Kip1 to cyclin D/CDK4 complexes leading to a redistribution and binding of p27Kip1 to cyclin E/CDK2 and cyclin A/CDK2 complexes with their inhibition.	bind
33228	6	7960	5	13	NULL	NULL	NULL	statement 1	Process	disruption of	leads to					statement 2	Process	redistribution of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_3_1091_s_239	11238057	37  These changes will disrupt binding of p27Kip1 to cyclin D/CDK4 complexes leading to a redistribution and binding of p27Kip1 to cyclin E/CDK2 and cyclin A/CDK2 complexes with their inhibition.	bind
33229	7	7960	5	13	NULL	NULL	NULL	statement 1	Process	disruption of	leads to					statement 3	Process	redistribution of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_3_1091_s_239	11238057	37  These changes will disrupt binding of p27Kip1 to cyclin D/CDK4 complexes leading to a redistribution and binding of p27Kip1 to cyclin E/CDK2 and cyclin A/CDK2 complexes with their inhibition.	bind
33230	8	7960	5	13	NULL	NULL	NULL	statement 2	Process		inhibits					cyclin E/cdk2 complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_3_1091_s_239	11238057	37  These changes will disrupt binding of p27Kip1 to cyclin D/CDK4 complexes leading to a redistribution and binding of p27Kip1 to cyclin E/CDK2 and cyclin A/CDK2 complexes with their inhibition.	bind
33231	9	7960	5	13	NULL	NULL	NULL	statement 3	Process		inhibits					cyclin A/CDK2 complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_3_1091_s_239	11238057	37  These changes will disrupt binding of p27Kip1 to cyclin D/CDK4 complexes leading to a redistribution and binding of p27Kip1 to cyclin E/CDK2 and cyclin A/CDK2 complexes with their inhibition.	bind
25572	1	7960	6	NULL	NULL	0	NULL	p27Kip1	NULL		bind	NULL				cyclin D/CDK4 complexes	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_3_1091_s_239	11238057	37  These changes will disrupt binding of p27Kip1 to cyclin D/CDK4 complexes leading to a redistribution and binding of p27Kip1 to cyclin E/CDK2 and cyclin A/CDK2 complexes with their inhibition.	bind
25573	2	7960	6	NULL	NULL	0	NULL	p27Kip1	NULL		bind	NULL				cyclin E/cdk2 complex	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_3_1091_s_239	11238057	37  These changes will disrupt binding of p27Kip1 to cyclin D/CDK4 complexes leading to a redistribution and binding of p27Kip1 to cyclin E/CDK2 and cyclin A/CDK2 complexes with their inhibition.	bind
25574	3	7960	6	NULL	NULL	0	NULL	p27Kip1	NULL		bind	NULL				cyclin A/CDK2 complex	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_3_1091_s_239	11238057	37  These changes will disrupt binding of p27Kip1 to cyclin D/CDK4 complexes leading to a redistribution and binding of p27Kip1 to cyclin E/CDK2 and cyclin A/CDK2 complexes with their inhibition.	bind
37375	4	7960	6	NULL	NULL	0	NULL	statement 1	NULL	disruption of	leads to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_3_1091_s_239	11238057	37  These changes will disrupt binding of p27Kip1 to cyclin D/CDK4 complexes leading to a redistribution and binding of p27Kip1 to cyclin E/CDK2 and cyclin A/CDK2 complexes with their inhibition.	bind
37377	5	7960	6	NULL	NULL	0	NULL	statement 1	NULL	disruption of	leads to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_3_1091_s_239	11238057	37  These changes will disrupt binding of p27Kip1 to cyclin D/CDK4 complexes leading to a redistribution and binding of p27Kip1 to cyclin E/CDK2 and cyclin A/CDK2 complexes with their inhibition.	bind
37379	6	7960	6	NULL	NULL	0	NULL	statement 1	NULL	disruption of	leads to	NULL				statement 2	NULL	redistribution of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_3_1091_s_239	11238057	37  These changes will disrupt binding of p27Kip1 to cyclin D/CDK4 complexes leading to a redistribution and binding of p27Kip1 to cyclin E/CDK2 and cyclin A/CDK2 complexes with their inhibition.	bind
37381	7	7960	6	NULL	NULL	0	NULL	statement 1	NULL	disruption of	leads to	NULL				statement 3	NULL	redistribution of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_3_1091_s_239	11238057	37  These changes will disrupt binding of p27Kip1 to cyclin D/CDK4 complexes leading to a redistribution and binding of p27Kip1 to cyclin E/CDK2 and cyclin A/CDK2 complexes with their inhibition.	bind
37382	8	7960	6	NULL	NULL	0	NULL	statement 2	NULL		inhibits	NULL				cyclin E/cdk2 complex	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_3_1091_s_239	11238057	37  These changes will disrupt binding of p27Kip1 to cyclin D/CDK4 complexes leading to a redistribution and binding of p27Kip1 to cyclin E/CDK2 and cyclin A/CDK2 complexes with their inhibition.	bind
37383	9	7960	6	NULL	NULL	0	NULL	statement 3	NULL		inhibits	NULL				cyclin A/CDK2 complex	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_3_1091_s_239	11238057	37  These changes will disrupt binding of p27Kip1 to cyclin D/CDK4 complexes leading to a redistribution and binding of p27Kip1 to cyclin E/CDK2 and cyclin A/CDK2 complexes with their inhibition.	bind
33234	1	7961	5	13	NULL	NULL	NULL	Lp(a)	GP		bind		weakly			LDL receptor	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_10_1774_s_172	7583555	37 38  Lp(a) binds weakly to the LDL receptor in vitro, 39  and LDL receptors probably play a minor role in the in vivo catabolism of Lp(a).	bind
33236	2	7961	5	13	NULL	NULL	NULL	LDL receptors	GP		plays a role in		probably;;minor			Lp(a)	GP	catabolism of			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_10_1774_s_172	7583555	37 38  Lp(a) binds weakly to the LDL receptor in vitro, 39  and LDL receptors probably play a minor role in the in vivo catabolism of Lp(a).	bind
25575	1	7961	6	NULL	NULL	0	NULL	Lp(a)	NULL		bind	NULL	weakly			LDL receptor	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_10_1774_s_172	7583555	37 38  Lp(a) binds weakly to the LDL receptor in vitro, 39  and LDL receptors probably play a minor role in the in vivo catabolism of Lp(a).	bind
25576	2	7961	6	10	NULL	0	NULL	LDL receptor	NULL		plays a role in	NULL	probably;; minor			Lp(a)	NULL	catabolism of 			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_10_1774_s_172	7583555	37 38  Lp(a) binds weakly to the LDL receptor in vitro, 39  and LDL receptors probably play a minor role in the in vivo catabolism of Lp(a).	bind
33237	1	7962	5	13	NULL	NULL	NULL	aspirin	Chemical		decreases					fibrinogen	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_3_363_s_112	11157686	37 38 39 40 41 42 43  The combination of aspirin plus an ADP antagonist decreases fibrinogen binding and platelet aggregation significantly more than either agent alone.	bind
33238	2	7962	5	13	NULL	NULL	NULL	aspirin	Chemical		decreases					platelet	Cell	aggregation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_3_363_s_112	11157686	37 38 39 40 41 42 43  The combination of aspirin plus an ADP antagonist decreases fibrinogen binding and platelet aggregation significantly more than either agent alone.	bind
49165	3	7962	5	13	NULL	NULL	NULL	ADP antagonist	Chemical		decreases					fibrinogen	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_3_363_s_112	11157686	37 38 39 40 41 42 43  The combination of aspirin plus an ADP antagonist decreases fibrinogen binding and platelet aggregation significantly more than either agent alone.	bind
49166	4	7962	5	13	NULL	NULL	NULL	ADP antagonist	Chemical		decreases					platelet	Cell	aggregation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_3_363_s_112	11157686	37 38 39 40 41 42 43  The combination of aspirin plus an ADP antagonist decreases fibrinogen binding and platelet aggregation significantly more than either agent alone.	bind
49167	5	7962	5	13	NULL	NULL	NULL	aspirin plus an ADP antagonist	Chemical		decreases					fibrinogen	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_3_363_s_112	11157686	37 38 39 40 41 42 43  The combination of aspirin plus an ADP antagonist decreases fibrinogen binding and platelet aggregation significantly more than either agent alone.	bind
49168	6	7962	5	13	NULL	NULL	NULL	aspirin plus an ADP antagonist	Chemical		decreases					platelet	Cell	aggregation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_3_363_s_112	11157686	37 38 39 40 41 42 43  The combination of aspirin plus an ADP antagonist decreases fibrinogen binding and platelet aggregation significantly more than either agent alone.	bind
49169	7	7962	5	13	NULL	NULL	NULL	statement 5	Process	efficiency of	is more than		significantly			statement 1	Process	efficiency of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_3_363_s_112	11157686	37 38 39 40 41 42 43  The combination of aspirin plus an ADP antagonist decreases fibrinogen binding and platelet aggregation significantly more than either agent alone.	bind
49170	8	7962	5	13	NULL	NULL	NULL	statement 5	Process	efficiency of	is more than		significantly			statement 3	Process	efficiency of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_3_363_s_112	11157686	37 38 39 40 41 42 43  The combination of aspirin plus an ADP antagonist decreases fibrinogen binding and platelet aggregation significantly more than either agent alone.	bind
49171	9	7962	5	13	NULL	NULL	NULL	statement 6	Process	efficiency of	is more than		significantly			statement 2	Process	efficiency of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_3_363_s_112	11157686	37 38 39 40 41 42 43  The combination of aspirin plus an ADP antagonist decreases fibrinogen binding and platelet aggregation significantly more than either agent alone.	bind
49172	10	7962	5	13	NULL	NULL	NULL	statement 6	Process	efficiency of	is more than		significantly			statement 4	Process	efficiency of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_3_363_s_112	11157686	37 38 39 40 41 42 43  The combination of aspirin plus an ADP antagonist decreases fibrinogen binding and platelet aggregation significantly more than either agent alone.	bind
25677	1	7962	6	NULL	NULL	0	NULL	aspirin	NULL		decreases	NULL				fibrinogen	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_circulation_103_3_363_s_112	11157686	37 38 39 40 41 42 43  The combination of aspirin plus an ADP antagonist decreases fibrinogen binding and platelet aggregation significantly more than either agent alone.	bind
25678	2	7962	6	NULL	NULL	0	NULL	aspirin	NULL		decreases	NULL				platelet	NULL	aggregation of			NULL		0	NULL	NULL	NULL	gw60_circulation_103_3_363_s_112	11157686	37 38 39 40 41 42 43  The combination of aspirin plus an ADP antagonist decreases fibrinogen binding and platelet aggregation significantly more than either agent alone.	bind
25679	3	7962	6	NULL	NULL	0	NULL	ADP antagonist	NULL		decreases	NULL				fibrinogen	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_circulation_103_3_363_s_112	11157686	37 38 39 40 41 42 43  The combination of aspirin plus an ADP antagonist decreases fibrinogen binding and platelet aggregation significantly more than either agent alone.	bind
25680	4	7962	6	NULL	NULL	0	NULL	ADP antagonist	NULL		decreases	NULL				platelet	NULL	aggregation of			NULL		0	NULL	NULL	NULL	gw60_circulation_103_3_363_s_112	11157686	37 38 39 40 41 42 43  The combination of aspirin plus an ADP antagonist decreases fibrinogen binding and platelet aggregation significantly more than either agent alone.	bind
25681	5	7962	6	NULL	NULL	0	NULL	aspirin plus an ADP antagonist	NULL		decreases	NULL				fibrinogen	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_circulation_103_3_363_s_112	11157686	37 38 39 40 41 42 43  The combination of aspirin plus an ADP antagonist decreases fibrinogen binding and platelet aggregation significantly more than either agent alone.	bind
25682	6	7962	6	NULL	NULL	0	NULL	aspirin plus an ADP antagonist	NULL		decreases	NULL				platelet	NULL	aggregation of			NULL		0	NULL	NULL	NULL	gw60_circulation_103_3_363_s_112	11157686	37 38 39 40 41 42 43  The combination of aspirin plus an ADP antagonist decreases fibrinogen binding and platelet aggregation significantly more than either agent alone.	bind
25683	7	7962	6	NULL	NULL	0	NULL	statement 5	NULL	efficiency of	is more	NULL	significantly			statement 1	NULL	efficiency of 			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_3_363_s_112	11157686	37 38 39 40 41 42 43  The combination of aspirin plus an ADP antagonist decreases fibrinogen binding and platelet aggregation significantly more than either agent alone.	bind
25684	8	7962	6	NULL	NULL	0	NULL	statement 5	NULL	efficiency of	is more	NULL	significantly			statement 3	NULL	efficiency of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_3_363_s_112	11157686	37 38 39 40 41 42 43  The combination of aspirin plus an ADP antagonist decreases fibrinogen binding and platelet aggregation significantly more than either agent alone.	bind
25685	9	7962	6	NULL	NULL	0	NULL	statement 6	NULL	efficiency of	is more	NULL	significantly			statement 2	NULL	efficiency of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_3_363_s_112	11157686	37 38 39 40 41 42 43  The combination of aspirin plus an ADP antagonist decreases fibrinogen binding and platelet aggregation significantly more than either agent alone.	bind
25686	10	7962	6	NULL	NULL	0	NULL	statement 6	NULL	efficiency of	is more	NULL	significantly			statement 4	NULL	efficiency of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_3_363_s_112	11157686	37 38 39 40 41 42 43  The combination of aspirin plus an ADP antagonist decreases fibrinogen binding and platelet aggregation significantly more than either agent alone.	bind
33384	1	7963	5	13	NULL	NULL	NULL	FXR	GP		modulate					ET-1	GP	expression of			NULL	EC	NULL	NULL	NULL	NULL	gw70_circulationres_98_2_192_s_235	16357303	37 FXR may similarly modulate ET-1 expression in EC via inhibition of AP-1 signaling as supported by the following observations: (1) pharmacological or genetic activation of FXR inhibited the activity of a heterologous promoter driven by AP-1 response elements ( Figure 7) and (2) FXR inhibited the binding of transcription factors to the AP-1 consensus site as shown in EMSA ( Figure 8A and 8B).	bind
33385	2	7963	5	13	NULL	NULL	NULL	statement 1	Process		via					AP-1 signaling	Process	inhibition of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_2_192_s_235	16357303	37 FXR may similarly modulate ET-1 expression in EC via inhibition of AP-1 signaling as supported by the following observations: (1) pharmacological or genetic activation of FXR inhibited the activity of a heterologous promoter driven by AP-1 response elements ( Figure 7) and (2) FXR inhibited the binding of transcription factors to the AP-1 consensus site as shown in EMSA ( Figure 8A and 8B).	bind
33386	3	7963	5	NULL	NULL	0	NULL		NULL		is driven by	NULL			heterologous promoter		NULL			AP-1 response elements	NULL		0	NULL	NULL	NULL	gw70_circulationres_98_2_192_s_235	16357303	37 FXR may similarly modulate ET-1 expression in EC via inhibition of AP-1 signaling as supported by the following observations: (1) pharmacological or genetic activation of FXR inhibited the activity of a heterologous promoter driven by AP-1 response elements ( Figure 7) and (2) FXR inhibited the binding of transcription factors to the AP-1 consensus site as shown in EMSA ( Figure 8A and 8B).	bind
33387	4	7963	5	13	NULL	NULL	NULL	FXR	GP	pharmacological activation of	inhibits					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_2_192_s_235	16357303	37 FXR may similarly modulate ET-1 expression in EC via inhibition of AP-1 signaling as supported by the following observations: (1) pharmacological or genetic activation of FXR inhibited the activity of a heterologous promoter driven by AP-1 response elements ( Figure 7) and (2) FXR inhibited the binding of transcription factors to the AP-1 consensus site as shown in EMSA ( Figure 8A and 8B).	bind
33388	5	7963	5	13	NULL	NULL	NULL	FXR	GP	genetic activation of	inhibits					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_2_192_s_235	16357303	37 FXR may similarly modulate ET-1 expression in EC via inhibition of AP-1 signaling as supported by the following observations: (1) pharmacological or genetic activation of FXR inhibited the activity of a heterologous promoter driven by AP-1 response elements ( Figure 7) and (2) FXR inhibited the binding of transcription factors to the AP-1 consensus site as shown in EMSA ( Figure 8A and 8B).	bind
33389	6	7963	5	13	NULL	NULL	NULL	statement 4	Process		is alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_2_192_s_235	16357303	37 FXR may similarly modulate ET-1 expression in EC via inhibition of AP-1 signaling as supported by the following observations: (1) pharmacological or genetic activation of FXR inhibited the activity of a heterologous promoter driven by AP-1 response elements ( Figure 7) and (2) FXR inhibited the binding of transcription factors to the AP-1 consensus site as shown in EMSA ( Figure 8A and 8B).	bind
33390	7	7963	5	13	NULL	NULL	NULL	transcription factors	GP		bind									AP-1 consensus site	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_2_192_s_235	16357303	37 FXR may similarly modulate ET-1 expression in EC via inhibition of AP-1 signaling as supported by the following observations: (1) pharmacological or genetic activation of FXR inhibited the activity of a heterologous promoter driven by AP-1 response elements ( Figure 7) and (2) FXR inhibited the binding of transcription factors to the AP-1 consensus site as shown in EMSA ( Figure 8A and 8B).	bind
33391	8	7963	5	13	NULL	NULL	NULL	FXR	GP		inhibits					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_2_192_s_235	16357303	37 FXR may similarly modulate ET-1 expression in EC via inhibition of AP-1 signaling as supported by the following observations: (1) pharmacological or genetic activation of FXR inhibited the activity of a heterologous promoter driven by AP-1 response elements ( Figure 7) and (2) FXR inhibited the binding of transcription factors to the AP-1 consensus site as shown in EMSA ( Figure 8A and 8B).	bind
25671	1	7963	6	NULL	NULL	0	NULL	heterologous promoter 	NULL		is driven by	NULL					NULL			AP-1 response element	NULL		0	NULL	NULL	NULL	gw70_circulationres_98_2_192_s_235	16357303	37 FXR may similarly modulate ET-1 expression in EC via inhibition of AP-1 signaling as supported by the following observations: (1) pharmacological or genetic activation of FXR inhibited the activity of a heterologous promoter driven by AP-1 response elements ( Figure 7) and (2) FXR inhibited the binding of transcription factors to the AP-1 consensus site as shown in EMSA ( Figure 8A and 8B).	bind
25672	2	7963	6	NULL	NULL	0	NULL	FXR	NULL	genetic activation of	inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_2_192_s_235	16357303	37 FXR may similarly modulate ET-1 expression in EC via inhibition of AP-1 signaling as supported by the following observations: (1) pharmacological or genetic activation of FXR inhibited the activity of a heterologous promoter driven by AP-1 response elements ( Figure 7) and (2) FXR inhibited the binding of transcription factors to the AP-1 consensus site as shown in EMSA ( Figure 8A and 8B).	bind
25673	3	7963	6	NULL	NULL	0	NULL	transcription factor	NULL		bind	NULL					NULL			AP-1 consensus site	NULL		0	NULL	NULL	NULL	gw70_circulationres_98_2_192_s_235	16357303	37 FXR may similarly modulate ET-1 expression in EC via inhibition of AP-1 signaling as supported by the following observations: (1) pharmacological or genetic activation of FXR inhibited the activity of a heterologous promoter driven by AP-1 response elements ( Figure 7) and (2) FXR inhibited the binding of transcription factors to the AP-1 consensus site as shown in EMSA ( Figure 8A and 8B).	bind
25674	4	7963	6	NULL	NULL	0	NULL	FXR	NULL		inhibits	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_2_192_s_235	16357303	37 FXR may similarly modulate ET-1 expression in EC via inhibition of AP-1 signaling as supported by the following observations: (1) pharmacological or genetic activation of FXR inhibited the activity of a heterologous promoter driven by AP-1 response elements ( Figure 7) and (2) FXR inhibited the binding of transcription factors to the AP-1 consensus site as shown in EMSA ( Figure 8A and 8B).	bind
48135	5	7963	6	10	NULL	0	NULL	FXR	NULL		modulate	NULL	may			ET-1	NULL	expression of			NULL	EC	0	NULL	NULL	NULL	gw70_circulationres_98_2_192_s_235	16357303	37 FXR may similarly modulate ET-1 expression in EC via inhibition of AP-1 signaling as supported by the following observations: (1) pharmacological or genetic activation of FXR inhibited the activity of a heterologous promoter driven by AP-1 response elements ( Figure 7) and (2) FXR inhibited the binding of transcription factors to the AP-1 consensus site as shown in EMSA ( Figure 8A and 8B).	bind
48136	6	7963	6	10	NULL	0	NULL	statement 5	NULL		occurs via	NULL				AP-1 signaling	NULL	inhibiton of			NULL		0	NULL	NULL	NULL	gw70_circulationres_98_2_192_s_235	16357303	37 FXR may similarly modulate ET-1 expression in EC via inhibition of AP-1 signaling as supported by the following observations: (1) pharmacological or genetic activation of FXR inhibited the activity of a heterologous promoter driven by AP-1 response elements ( Figure 7) and (2) FXR inhibited the binding of transcription factors to the AP-1 consensus site as shown in EMSA ( Figure 8A and 8B).	bind
48137	7	7963	6	10	NULL	0	NULL	FXR	NULL	pharmacological activation of	inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_2_192_s_235	16357303	37 FXR may similarly modulate ET-1 expression in EC via inhibition of AP-1 signaling as supported by the following observations: (1) pharmacological or genetic activation of FXR inhibited the activity of a heterologous promoter driven by AP-1 response elements ( Figure 7) and (2) FXR inhibited the binding of transcription factors to the AP-1 consensus site as shown in EMSA ( Figure 8A and 8B).	bind
48138	8	7963	6	10	NULL	0	NULL	statement 2	NULL		is an alternative to	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_2_192_s_235	16357303	37 FXR may similarly modulate ET-1 expression in EC via inhibition of AP-1 signaling as supported by the following observations: (1) pharmacological or genetic activation of FXR inhibited the activity of a heterologous promoter driven by AP-1 response elements ( Figure 7) and (2) FXR inhibited the binding of transcription factors to the AP-1 consensus site as shown in EMSA ( Figure 8A and 8B).	bind
33241	1	7964	5	13	NULL	NULL	NULL	A20	GP		bind					IKKgamma/NEMO	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_6_630_s_203	12609966	37 Interestingly, binding of A20 alone to IKKgamma/NEMO is not sufficient to inhibit NF-kappaB, suggesting possible involvement of additional molecules.	bind
33242	2	7964	5	13	NULL	NULL	NULL	statement 1	Process		does not inhibit					NF-kappaB	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_6_630_s_203	12609966	37 Interestingly, binding of A20 alone to IKKgamma/NEMO is not sufficient to inhibit NF-kappaB, suggesting possible involvement of additional molecules.	bind
25577	1	7964	6	NULL	NULL	0	NULL	A20	NULL		bind	NULL				IKKgamma/NEMO	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_92_6_630_s_203	12609966	37 Interestingly, binding of A20 alone to IKKgamma/NEMO is not sufficient to inhibit NF-kappaB, suggesting possible involvement of additional molecules.	bind
25578	2	7964	6	NULL	NULL	0	NULL	statement 1	NULL		does not inhibit	NULL				NF-kappaB	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_6_630_s_203	12609966	37 Interestingly, binding of A20 alone to IKKgamma/NEMO is not sufficient to inhibit NF-kappaB, suggesting possible involvement of additional molecules.	bind
33239	1	7965	5	13	NULL	NULL	NULL	TSP1	GP		bind					TGF-beta1	GP	latent			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_3_831_s_248	12213711	37 Recent studies have shown that TSP1 binds and activates latent TGF-beta1.	bind
33240	2	7965	5	13	NULL	NULL	NULL	statement 1	Process		activates					TGF-beta1	GP	latent			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_3_831_s_248	12213711	37 Recent studies have shown that TSP1 binds and activates latent TGF-beta1.	bind
25579	1	7965	6	NULL	NULL	0	NULL	TSP1	NULL		bind	NULL				TGF-beta1	NULL	latent			NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_3_831_s_248	12213711	37 Recent studies have shown that TSP1 binds and activates latent TGF-beta1.	bind
25580	2	7965	6	NULL	NULL	0	NULL	TSP1	NULL		activates	NULL				TGF-beta1	NULL	latent			NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_3_831_s_248	12213711	37 Recent studies have shown that TSP1 binds and activates latent TGF-beta1.	bind
37881	3	7965	6	NULL	NULL	0	NULL	statement 1	NULL		occurs simultaneously with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_3_831_s_248	12213711	37 Recent studies have shown that TSP1 binds and activates latent TGF-beta1.	bind
33244	1	7966	5	13	NULL	NULL	NULL	gp120	GP		is a type of					HIV-1 envelope protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_5_1631_s_243	9811356	37, 39 In cultured human fetal neurons, CD4-independent binding of the HIV-1 envelope protein gp120 to CXCR4 was recently reported.	bind
33245	2	7966	5	13	NULL	NULL	NULL	gp120	GP		bind					CXCR4	GP				NULL	cultured human fetal neurons	NULL	NULL	NULL	NULL	gw60_amjpathol_153_5_1631_s_243	9811356	37, 39 In cultured human fetal neurons, CD4-independent binding of the HIV-1 envelope protein gp120 to CXCR4 was recently reported.	bind
33247	3	7966	5	13	NULL	NULL	NULL	statement 2	Process		is independent of					CD4	GP				NULL	cultured human fetal neurons	NULL	NULL	NULL	NULL	gw60_amjpathol_153_5_1631_s_243	9811356	37, 39 In cultured human fetal neurons, CD4-independent binding of the HIV-1 envelope protein gp120 to CXCR4 was recently reported.	bind
25581	1	7966	6	NULL	NULL	0	NULL	gp120	NULL		bind	NULL				CXCR4	NULL				NULL	cultured human fetal neurons	NULL	NULL	NULL	NULL	gw60_amjpathol_153_5_1631_s_243	9811356	37, 39 In cultured human fetal neurons, CD4-independent binding of the HIV-1 envelope protein gp120 to CXCR4 was recently reported.	bind
25582	2	7966	6	10	NULL	0	NULL	statement 1			is independent of					CD4					NULL	cultured human fetal neurons	NULL	NULL	NULL	NULL	gw60_amjpathol_153_5_1631_s_243	9811356	37, 39 In cultured human fetal neurons, CD4-independent binding of the HIV-1 envelope protein gp120 to CXCR4 was recently reported.	bind
37388	3	7966	6	NULL	NULL	0	NULL	gp120	NULL		is a type of	NULL				HIV-1 envelope protein	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_5_1631_s_243	9811356	37, 39 In cultured human fetal neurons, CD4-independent binding of the HIV-1 envelope protein gp120 to CXCR4 was recently reported.	bind
33350	1	7967	5	13	NULL	NULL	NULL	E-selectin gene	GP	endothelial	contain		may			NF-kappaB	GP			DNA-binding sequences	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2075_s_174	15374848	37,38  Furthermore, endothelial E-selectin gene may present DNA-binding sequences for both NF-kappaB and AP-1, 39 and multiple NF-kappaB binding sites in the human E-selectin gene are required for maximal TNF-alpha - induced expression.	bind
33354	2	7967	5	13	NULL	NULL	NULL	E-selectin gene	GP	endothelial	contain		may			AP-1	GP			DNA-binding sequences	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2075_s_174	15374848	37,38  Furthermore, endothelial E-selectin gene may present DNA-binding sequences for both NF-kappaB and AP-1, 39 and multiple NF-kappaB binding sites in the human E-selectin gene are required for maximal TNF-alpha - induced expression.	bind
33355	4	7967	5	13	NULL	NULL	NULL	E-selectin gene	GP	human	is required for				multiple NF-kappaB binding sites	statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2075_s_174	15374848	37,38  Furthermore, endothelial E-selectin gene may present DNA-binding sequences for both NF-kappaB and AP-1, 39 and multiple NF-kappaB binding sites in the human E-selectin gene are required for maximal TNF-alpha - induced expression.	bind
47833	3	7967	5	13	NULL	NULL	NULL	TNF-alpha	GP		induce					expression	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2075_s_174	15374848	37,38  Furthermore, endothelial E-selectin gene may present DNA-binding sequences for both NF-kappaB and AP-1, 39 and multiple NF-kappaB binding sites in the human E-selectin gene are required for maximal TNF-alpha - induced expression.	bind
25583	4	7967	6	10	NULL	0	NULL	E-selectin gene	NULL	human	is required for	NULL			NF-kappaB binding sites	statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2075_s_174	15374848	37,38  Furthermore, endothelial E-selectin gene may present DNA-binding sequences for both NF-kappaB and AP-1, 39 and multiple NF-kappaB binding sites in the human E-selectin gene are required for maximal TNF-alpha - induced expression.	bind
37389	2	7967	6	NULL	NULL	0	NULL	E-selectin gene	NULL	endothelial	contain	NULL	may			NF-kappaB	NULL			DNA binding sequences	NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2075_s_174	15374848	37,38  Furthermore, endothelial E-selectin gene may present DNA-binding sequences for both NF-kappaB and AP-1, 39 and multiple NF-kappaB binding sites in the human E-selectin gene are required for maximal TNF-alpha - induced expression.	bind
37391	1	7967	6	10	NULL	0	NULL	E-selectin gene	NULL	endothelial	contain	NULL	may			AP-1	NULL			DNA binding sequences	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2075_s_174	15374848	37,38  Furthermore, endothelial E-selectin gene may present DNA-binding sequences for both NF-kappaB and AP-1, 39 and multiple NF-kappaB binding sites in the human E-selectin gene are required for maximal TNF-alpha - induced expression.	bind
47834	3	7967	6	10	NULL	0	NULL	TNF-alpha	NULL		induce	NULL				expression	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2075_s_174	15374848	37,38  Furthermore, endothelial E-selectin gene may present DNA-binding sequences for both NF-kappaB and AP-1, 39 and multiple NF-kappaB binding sites in the human E-selectin gene are required for maximal TNF-alpha - induced expression.	bind
33358	1	7968	5	13	NULL	NULL	NULL	estrogen	Chemical		bind					membrane receptors	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_2_245_s_157	14670845	37,38  Previous studies demonstrated that after estrogen binds to membrane receptors, followed by the activation of G proteins, 34 multiple signaling pathways that have been linked to either the stimulation of gene transcription or posttranslational modification of proteins, 39 - 41   are rapidly activated.	bind
33360	2	7968	5	13	NULL	NULL	NULL	statement 1	Process		followed by					G proteins	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_2_245_s_157	14670845	37,38  Previous studies demonstrated that after estrogen binds to membrane receptors, followed by the activation of G proteins, 34 multiple signaling pathways that have been linked to either the stimulation of gene transcription or posttranslational modification of proteins, 39 - 41   are rapidly activated.	bind
33361	3	7968	5	13	NULL	NULL	NULL	signaling pathways	Process	multiple	stimulates					gene transcription	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_2_245_s_157	14670845	37,38  Previous studies demonstrated that after estrogen binds to membrane receptors, followed by the activation of G proteins, 34 multiple signaling pathways that have been linked to either the stimulation of gene transcription or posttranslational modification of proteins, 39 - 41   are rapidly activated.	bind
33362	4	7968	5	13	NULL	NULL	NULL	signaling pathways	Process	multiple	stimulates					proteins	GP	posttranslational modification of 			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_2_245_s_157	14670845	37,38  Previous studies demonstrated that after estrogen binds to membrane receptors, followed by the activation of G proteins, 34 multiple signaling pathways that have been linked to either the stimulation of gene transcription or posttranslational modification of proteins, 39 - 41   are rapidly activated.	bind
33363	5	7968	5	13	NULL	NULL	NULL	statement 2	Process		activates		rapidly			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_2_245_s_157	14670845	37,38  Previous studies demonstrated that after estrogen binds to membrane receptors, followed by the activation of G proteins, 34 multiple signaling pathways that have been linked to either the stimulation of gene transcription or posttranslational modification of proteins, 39 - 41   are rapidly activated.	bind
33364	6	7968	5	13	NULL	NULL	NULL	statement 2	Process		activates		rapidly			statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_2_245_s_157	14670845	37,38  Previous studies demonstrated that after estrogen binds to membrane receptors, followed by the activation of G proteins, 34 multiple signaling pathways that have been linked to either the stimulation of gene transcription or posttranslational modification of proteins, 39 - 41   are rapidly activated.	bind
25589	1	7968	6	NULL	NULL	0	NULL	estrogen	NULL		bind	NULL				membrane receptors	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_2_245_s_157	14670845	37,38  Previous studies demonstrated that after estrogen binds to membrane receptors, followed by the activation of G proteins, 34 multiple signaling pathways that have been linked to either the stimulation of gene transcription or posttranslational modification of proteins, 39 - 41   are rapidly activated.	bind
25590	2	7968	6	NULL	NULL	0	NULL	statement 1	NULL		activates	NULL				G proteins	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_2_245_s_157	14670845	37,38  Previous studies demonstrated that after estrogen binds to membrane receptors, followed by the activation of G proteins, 34 multiple signaling pathways that have been linked to either the stimulation of gene transcription or posttranslational modification of proteins, 39 - 41   are rapidly activated.	bind
25591	3	7968	6	NULL	NULL	0	NULL	signaling pathways	NULL		linked to	NULL				gene transcription	NULL	stimulation of			NULL		0	NULL	NULL	NULL	gw70_circulationres_94_2_245_s_157	14670845	37,38  Previous studies demonstrated that after estrogen binds to membrane receptors, followed by the activation of G proteins, 34 multiple signaling pathways that have been linked to either the stimulation of gene transcription or posttranslational modification of proteins, 39 - 41   are rapidly activated.	bind
25592	4	7968	6	NULL	NULL	0	NULL	signaling pathways	NULL		linked to	NULL				proteins	NULL	posttranslational modification of			NULL		0	NULL	NULL	NULL	gw70_circulationres_94_2_245_s_157	14670845	37,38  Previous studies demonstrated that after estrogen binds to membrane receptors, followed by the activation of G proteins, 34 multiple signaling pathways that have been linked to either the stimulation of gene transcription or posttranslational modification of proteins, 39 - 41   are rapidly activated.	bind
25593	5	7968	6	NULL	NULL	0	NULL	statement 1	NULL		activates	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_2_245_s_157	14670845	37,38  Previous studies demonstrated that after estrogen binds to membrane receptors, followed by the activation of G proteins, 34 multiple signaling pathways that have been linked to either the stimulation of gene transcription or posttranslational modification of proteins, 39 - 41   are rapidly activated.	bind
25594	6	7968	6	NULL	NULL	0	NULL	statement 1	NULL		activates	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_2_245_s_157	14670845	37,38  Previous studies demonstrated that after estrogen binds to membrane receptors, followed by the activation of G proteins, 34 multiple signaling pathways that have been linked to either the stimulation of gene transcription or posttranslational modification of proteins, 39 - 41   are rapidly activated.	bind
33365	1	7969	5	13	NULL	NULL	NULL	PKC	GP		enhances					NF-kappaB	GP	activity of			NULL	C pneumoniae - infected HAECs	NULL	NULL	NULL	NULL	gw60_circulationres_92_10_1130_s_200	12714566	37,41  Hence, in  C pneumoniae - infected HAECs, we demonstrate that PKC enhances NF-kappaB activity by direct phosphorylation of its cytoplasmic inhibitor, I-kappaBalpha, thus facilitating NF-kappaB binding to the NF-kappaB motif in the ICAM-1 promoter.	bind
33368	2	7969	5	13	NULL	NULL	NULL	PKC	GP		phosphorylates		directly			I-kappaBalpha	GP				NULL	C pneumoniae - infected HAECs	NULL	NULL	NULL	NULL	gw60_circulationres_92_10_1130_s_200	12714566	37,41  Hence, in  C pneumoniae - infected HAECs, we demonstrate that PKC enhances NF-kappaB activity by direct phosphorylation of its cytoplasmic inhibitor, I-kappaBalpha, thus facilitating NF-kappaB binding to the NF-kappaB motif in the ICAM-1 promoter.	bind
33370	3	7969	5	13	NULL	NULL	NULL	I-kappaBalpha	GP		inhibit					NF-kappaB	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_10_1130_s_200	12714566	37,41  Hence, in  C pneumoniae - infected HAECs, we demonstrate that PKC enhances NF-kappaB activity by direct phosphorylation of its cytoplasmic inhibitor, I-kappaBalpha, thus facilitating NF-kappaB binding to the NF-kappaB motif in the ICAM-1 promoter.	bind
33371	4	7969	5	13	NULL	NULL	NULL	NF-kappaB	GP		bind					ICAM-1	GP			NF-kappaB motif in promoter	NULL	C pneumoniae - infected HAECs	NULL	NULL	NULL	NULL	gw60_circulationres_92_10_1130_s_200	12714566	37,41  Hence, in  C pneumoniae - infected HAECs, we demonstrate that PKC enhances NF-kappaB activity by direct phosphorylation of its cytoplasmic inhibitor, I-kappaBalpha, thus facilitating NF-kappaB binding to the NF-kappaB motif in the ICAM-1 promoter.	bind
33373	5	7969	5	13	NULL	NULL	NULL	statement 1	Process		facilitate					statement 4	Process				NULL	C pneumoniae - infected HAECs	NULL	NULL	NULL	NULL	gw60_circulationres_92_10_1130_s_200	12714566	37,41  Hence, in  C pneumoniae - infected HAECs, we demonstrate that PKC enhances NF-kappaB activity by direct phosphorylation of its cytoplasmic inhibitor, I-kappaBalpha, thus facilitating NF-kappaB binding to the NF-kappaB motif in the ICAM-1 promoter.	bind
36175	6	7969	5	13	NULL	NULL	NULL	I-kappaBalpha	GP		is a type of					cytoplasmic inhibitor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_10_1130_s_200	12714566	37,41  Hence, in  C pneumoniae - infected HAECs, we demonstrate that PKC enhances NF-kappaB activity by direct phosphorylation of its cytoplasmic inhibitor, I-kappaBalpha, thus facilitating NF-kappaB binding to the NF-kappaB motif in the ICAM-1 promoter.	bind
25584	1	7969	6	10	NULL	0	NULL	PKC	NULL		phosphorylates	NULL	directly			I-kappaBalpha	NULL				NULL	C pneumoniae - infected HAEC	NULL	NULL	NULL	NULL	gw60_circulationres_92_10_1130_s_200	12714566	37,41  Hence, in  C pneumoniae - infected HAECs, we demonstrate that PKC enhances NF-kappaB activity by direct phosphorylation of its cytoplasmic inhibitor, I-kappaBalpha, thus facilitating NF-kappaB binding to the NF-kappaB motif in the ICAM-1 promoter.	bind
25585	2	7969	6	NULL	NULL	0	NULL	PKC	NULL		enhances	NULL				NF-kappaB	NULL	activity of			NULL	C pneumoniae - infected HAEC	NULL	NULL	NULL	NULL	gw60_circulationres_92_10_1130_s_200	12714566	37,41  Hence, in  C pneumoniae - infected HAECs, we demonstrate that PKC enhances NF-kappaB activity by direct phosphorylation of its cytoplasmic inhibitor, I-kappaBalpha, thus facilitating NF-kappaB binding to the NF-kappaB motif in the ICAM-1 promoter.	bind
25586	3	7969	6	NULL	NULL	0	NULL	statement 2	NULL		occurs via	NULL				statement 1	NULL				NULL	C pneumoniae - infected HAEC	NULL	NULL	NULL	NULL	gw60_circulationres_92_10_1130_s_200	12714566	37,41  Hence, in  C pneumoniae - infected HAECs, we demonstrate that PKC enhances NF-kappaB activity by direct phosphorylation of its cytoplasmic inhibitor, I-kappaBalpha, thus facilitating NF-kappaB binding to the NF-kappaB motif in the ICAM-1 promoter.	bind
25587	4	7969	6	NULL	NULL	0	NULL	NF-kappaB	NULL		bind	NULL				ICAM-1	NULL			NF-kappaB motif of the promoter	NULL	C pneumoniae - infected HAEC	NULL	NULL	NULL	NULL	gw60_circulationres_92_10_1130_s_200	12714566	37,41  Hence, in  C pneumoniae - infected HAECs, we demonstrate that PKC enhances NF-kappaB activity by direct phosphorylation of its cytoplasmic inhibitor, I-kappaBalpha, thus facilitating NF-kappaB binding to the NF-kappaB motif in the ICAM-1 promoter.	bind
25588	5	7969	6	NULL	NULL	0	NULL	statement 2	NULL		facilitate	NULL				statement 4	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_10_1130_s_200	12714566	37,41  Hence, in  C pneumoniae - infected HAECs, we demonstrate that PKC enhances NF-kappaB activity by direct phosphorylation of its cytoplasmic inhibitor, I-kappaBalpha, thus facilitating NF-kappaB binding to the NF-kappaB motif in the ICAM-1 promoter.	bind
37393	6	7969	6	NULL	NULL	0	NULL	I-kappaBalpha	NULL		is a type of	NULL				cytoplasmic inhibitor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_92_10_1130_s_200	12714566	37,41  Hence, in  C pneumoniae - infected HAECs, we demonstrate that PKC enhances NF-kappaB activity by direct phosphorylation of its cytoplasmic inhibitor, I-kappaBalpha, thus facilitating NF-kappaB binding to the NF-kappaB motif in the ICAM-1 promoter.	bind
37394	7	7969	6	NULL	NULL	0	NULL	IkappaBalpha	NULL		inhibits	NULL				NF-kappaB	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_92_10_1130_s_200	12714566	37,41  Hence, in  C pneumoniae - infected HAECs, we demonstrate that PKC enhances NF-kappaB activity by direct phosphorylation of its cytoplasmic inhibitor, I-kappaBalpha, thus facilitating NF-kappaB binding to the NF-kappaB motif in the ICAM-1 promoter.	bind
33376	1	7970	5	13	NULL	NULL	NULL	GST fusion protein	GP	bait	contains					SHP-2	GP		tandem SH2 domains		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_63	12689916	37,41,45,46,48,50,54,57 - 59           Interestingly, in a completely unbiased approach, a bait GST fusion protein containing the tandem SH2 domains of SHP-2 exclusively bound a peptide comprised of PECAM-1 residues 617 to 711 (ie, containing its dual ITIM), when tyrosine-phosphorylated, out of an entire phage display cDNA library.	bind
33377	2	7970	5	13	NULL	NULL	NULL	statement 1	Process		bind					PECAM-1 peptide	GP		residues 617 to 711		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_63	12689916	37,41,45,46,48,50,54,57 - 59           Interestingly, in a completely unbiased approach, a bait GST fusion protein containing the tandem SH2 domains of SHP-2 exclusively bound a peptide comprised of PECAM-1 residues 617 to 711 (ie, containing its dual ITIM), when tyrosine-phosphorylated, out of an entire phage display cDNA library.	bind
33379	3	7970	5	13	NULL	NULL	NULL	PECAM-1 peptide	GP		contains			residues 617 to 711					dual ITIM		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_63	12689916	37,41,45,46,48,50,54,57 - 59           Interestingly, in a completely unbiased approach, a bait GST fusion protein containing the tandem SH2 domains of SHP-2 exclusively bound a peptide comprised of PECAM-1 residues 617 to 711 (ie, containing its dual ITIM), when tyrosine-phosphorylated, out of an entire phage display cDNA library.	bind
33380	4	7970	5	13	NULL	NULL	NULL	tyrosine	AminoAcid	phosphorylation of	is required for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_63	12689916	37,41,45,46,48,50,54,57 - 59           Interestingly, in a completely unbiased approach, a bait GST fusion protein containing the tandem SH2 domains of SHP-2 exclusively bound a peptide comprised of PECAM-1 residues 617 to 711 (ie, containing its dual ITIM), when tyrosine-phosphorylated, out of an entire phage display cDNA library.	bind
26257	1	7970	6	NULL	NULL	0	NULL	GST fusion protein	NULL		contains	NULL				SHP-2	NULL		tandem SH2 domains		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_63	12689916	37,41,45,46,48,50,54,57 - 59           Interestingly, in a completely unbiased approach, a bait GST fusion protein containing the tandem SH2 domains of SHP-2 exclusively bound a peptide comprised of PECAM-1 residues 617 to 711 (ie, containing its dual ITIM), when tyrosine-phosphorylated, out of an entire phage display cDNA library.	bind
26258	2	7970	6	NULL	NULL	0	NULL	peptide	NULL		comprises of	NULL				PECAM-1	NULL		residues 617-711		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_63	12689916	37,41,45,46,48,50,54,57 - 59           Interestingly, in a completely unbiased approach, a bait GST fusion protein containing the tandem SH2 domains of SHP-2 exclusively bound a peptide comprised of PECAM-1 residues 617 to 711 (ie, containing its dual ITIM), when tyrosine-phosphorylated, out of an entire phage display cDNA library.	bind
26259	3	7970	6	NULL	NULL	0	NULL	GST fusion protein	NULL	phosphorylated	bind	NULL		tyrosine		statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_63	12689916	37,41,45,46,48,50,54,57 - 59           Interestingly, in a completely unbiased approach, a bait GST fusion protein containing the tandem SH2 domains of SHP-2 exclusively bound a peptide comprised of PECAM-1 residues 617 to 711 (ie, containing its dual ITIM), when tyrosine-phosphorylated, out of an entire phage display cDNA library.	bind
37396	4	7970	6	NULL	NULL	0	NULL	PECAM-1	NULL		contains	NULL		residues 617-711		dual ITIM	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_63	12689916	37,41,45,46,48,50,54,57 - 59           Interestingly, in a completely unbiased approach, a bait GST fusion protein containing the tandem SH2 domains of SHP-2 exclusively bound a peptide comprised of PECAM-1 residues 617 to 711 (ie, containing its dual ITIM), when tyrosine-phosphorylated, out of an entire phage display cDNA library.	bind
33393	1	7971	5	13	NULL	NULL	NULL				bind		directly	amphipathic helices		ABCA1	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_j-lipid-res_47_1_16210729_s_6	16210729	37pA was cross-linked  to ABCA1, confirming the direct binding of amphipathic helices to ABCA1.	bind
25863	1	7971	6	NULL	NULL	0	NULL		NULL		bind	NULL	directly	amphipathic helices		ABCA1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0570-0579_j-lipid-res_47_1_16210729_s_6	16210729	37pA was cross-linked  to ABCA1, confirming the direct binding of amphipathic helices to ABCA1.	bind
33395	1	7973	5	13	NULL	NULL	NULL	Tb(III)	GP		bind					hammerhead ribozyme	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_22_4428_s_347	11071929	38       Feig,A.L., Panek,M., Horrocks,W.D. and Uhlenbeck,O.C. (1999) Probing the binding of Tb(III) and Eu(III) to the hammerhead ribozyme using luminescence spectroscopy.	bind
33396	2	7973	5	13	NULL	NULL	NULL	Eu(III)	GP		bind					hammerhead ribozyme	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_22_4428_s_347	11071929	38       Feig,A.L., Panek,M., Horrocks,W.D. and Uhlenbeck,O.C. (1999) Probing the binding of Tb(III) and Eu(III) to the hammerhead ribozyme using luminescence spectroscopy.	bind
25864	1	7973	6	NULL	NULL	0	NULL	Tb(III)	NULL		bind	NULL				hammerhead ribozyme	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_22_4428_s_347	11071929	38       Feig,A.L., Panek,M., Horrocks,W.D. and Uhlenbeck,O.C. (1999) Probing the binding of Tb(III) and Eu(III) to the hammerhead ribozyme using luminescence spectroscopy.	bind
25865	2	7973	6	NULL	NULL	0	NULL	Eu(III)	NULL		bind	NULL				hammerhead ribozyme	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_22_4428_s_347	11071929	38       Feig,A.L., Panek,M., Horrocks,W.D. and Uhlenbeck,O.C. (1999) Probing the binding of Tb(III) and Eu(III) to the hammerhead ribozyme using luminescence spectroscopy.	bind
33397	1	7975	5	13	NULL	NULL	NULL	nuclear proteins	GP	rice	bind		sequence specifically;; independently					rice bacilliform virus		vascular bundle expression element	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_497_s_399	11788712	38       He,X., Futterer,J. and Hohn,T. (2001) Sequence specific, methylation dependent and independent binding of rice nuclear proteins to a rice bacilliform virus vascular bundle expression element  J. Biol.	bind
36174	2	7975	5	13	NULL	NULL	NULL	statement 1	Process		is dependent on					methylation	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_497_s_399	11788712	38       He,X., Futterer,J. and Hohn,T. (2001) Sequence specific, methylation dependent and independent binding of rice nuclear proteins to a rice bacilliform virus vascular bundle expression element  J. Biol.	bind
25866	1	7975	6	NULL	NULL	0	NULL	nuclear proteins	NULL	rice	bind	NULL	sequence specifically;; independently				NULL	rice bacilliform virus		vascular bundle expression element	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_497_s_399	11788712	38       He,X., Futterer,J. and Hohn,T. (2001) Sequence specific, methylation dependent and independent binding of rice nuclear proteins to a rice bacilliform virus vascular bundle expression element  J. Biol.	bind
25867	2	7975	6	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				methylation	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_497_s_399	11788712	38       He,X., Futterer,J. and Hohn,T. (2001) Sequence specific, methylation dependent and independent binding of rice nuclear proteins to a rice bacilliform virus vascular bundle expression element  J. Biol.	bind
33398	1	7976	5	13	NULL	NULL	NULL	U1A protein	GP		bind		high affinity			U1 hairpin II RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_550_s_375	11788718	38       Katsamba,P.S., Myszka,D.G. and Laird-Offringa,I.A. (2001) Two functionally distinct steps mediate high affinity binding of U1A protein to U1 hairpin II RNA.	bind
25868	1	7976	6	NULL	NULL	0	NULL	U1A protein	NULL		bind	NULL	high affinity			U1 hairpin II RNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_550_s_375	11788718	38       Katsamba,P.S., Myszka,D.G. and Laird-Offringa,I.A. (2001) Two functionally distinct steps mediate high affinity binding of U1A protein to U1 hairpin II RNA.	bind
33399	1	7977	5	13	NULL	NULL	NULL	nuclear protein	GP		bind					Ki-ras	GP	human		promoter	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_622_s_325	11160882	38       Mayfield,C., Squibb,M. and Miller,D. (1994) Inhibition of nuclear protein binding to the human Ki-ras promoter by triplex-forming oligonucleotides.	bind
33400	2	7977	5	13	NULL	NULL	NULL	oligonucleotides	NucleicAcid	triplex-forming	inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_622_s_325	11160882	38       Mayfield,C., Squibb,M. and Miller,D. (1994) Inhibition of nuclear protein binding to the human Ki-ras promoter by triplex-forming oligonucleotides.	bind
25869	1	7977	6	NULL	NULL	0	NULL	nuclear protein	NULL		bind	NULL				Ki-ras	NULL	human		promoter	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_622_s_325	11160882	38       Mayfield,C., Squibb,M. and Miller,D. (1994) Inhibition of nuclear protein binding to the human Ki-ras promoter by triplex-forming oligonucleotides.	bind
25870	2	7977	6	NULL	NULL	0	NULL	oligonucleotides	NULL	triplex-forming	inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_622_s_325	11160882	38       Mayfield,C., Squibb,M. and Miller,D. (1994) Inhibition of nuclear protein binding to the human Ki-ras promoter by triplex-forming oligonucleotides.	bind
33401	1	7979	5	13	NULL	NULL	NULL	LDL	GP		bind					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_9_1287_s_72	7670940	38  Antibody B1B3 54  but not antibody D7.2 37  inhibits the binding of LDL to the LDL receptor.	bind
33402	2	7979	5	13	NULL	NULL	NULL	antibody B1B3 54	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_9_1287_s_72	7670940	38  Antibody B1B3 54  but not antibody D7.2 37  inhibits the binding of LDL to the LDL receptor.	bind
33403	3	7979	5	13	NULL	NULL	NULL	antibody D7.2 37	GP		does not inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_9_1287_s_72	7670940	38  Antibody B1B3 54  but not antibody D7.2 37  inhibits the binding of LDL to the LDL receptor.	bind
25871	1	7979	6	NULL	NULL	0	NULL	LDL	NULL		bind	NULL				LDL receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_9_1287_s_72	7670940	38  Antibody B1B3 54  but not antibody D7.2 37  inhibits the binding of LDL to the LDL receptor.	bind
25872	2	7979	6	NULL	NULL	0	NULL	Antibody B1B3	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_9_1287_s_72	7670940	38  Antibody B1B3 54  but not antibody D7.2 37  inhibits the binding of LDL to the LDL receptor.	bind
25873	3	7979	6	NULL	NULL	0	NULL	antibody D7.2	NULL		does not inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_9_1287_s_72	7670940	38  Antibody B1B3 54  but not antibody D7.2 37  inhibits the binding of LDL to the LDL receptor.	bind
33404	1	7980	5	13	NULL	NULL	NULL	LDL	GP	oxidation of	is a critical process in					atherogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1375_s_135	7867176	38  Furthermore, oxidation of LDL, now thought to be a critical process in atherogenesis, 39  increases binding of LDL to collagen, 40  raising the possibility of damage to collagen or elastin fibers mediated by free radicals derived from lipid hydroperoxides and other reactive intermediaries.	bind
33405	2	7980	5	13	NULL	NULL	NULL	LDL	GP		bind					collagen	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1375_s_135	7867176	38  Furthermore, oxidation of LDL, now thought to be a critical process in atherogenesis, 39  increases binding of LDL to collagen, 40  raising the possibility of damage to collagen or elastin fibers mediated by free radicals derived from lipid hydroperoxides and other reactive intermediaries.	bind
33406	3	7980	5	13	NULL	NULL	NULL	LDL	GP	oxidation of	increases					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1375_s_135	7867176	38  Furthermore, oxidation of LDL, now thought to be a critical process in atherogenesis, 39  increases binding of LDL to collagen, 40  raising the possibility of damage to collagen or elastin fibers mediated by free radicals derived from lipid hydroperoxides and other reactive intermediaries.	bind
33407	4	7980	5	13	NULL	NULL	NULL	free radicals	Chemical		derived from					lipid hydroperoxides	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1375_s_135	7867176	38  Furthermore, oxidation of LDL, now thought to be a critical process in atherogenesis, 39  increases binding of LDL to collagen, 40  raising the possibility of damage to collagen or elastin fibers mediated by free radicals derived from lipid hydroperoxides and other reactive intermediaries.	bind
33408	5	7980	5	13	NULL	NULL	NULL	free radicals	Chemical		derived from					intermediaries	Chemical	reactive			NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1375_s_135	7867176	38  Furthermore, oxidation of LDL, now thought to be a critical process in atherogenesis, 39  increases binding of LDL to collagen, 40  raising the possibility of damage to collagen or elastin fibers mediated by free radicals derived from lipid hydroperoxides and other reactive intermediaries.	bind
33409	6	7980	5	13	NULL	NULL	NULL	statement 3	Process		damages		possibly			collagen fibers	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1375_s_135	7867176	38  Furthermore, oxidation of LDL, now thought to be a critical process in atherogenesis, 39  increases binding of LDL to collagen, 40  raising the possibility of damage to collagen or elastin fibers mediated by free radicals derived from lipid hydroperoxides and other reactive intermediaries.	bind
33410	7	7980	5	13	NULL	NULL	NULL	statement 4	Process		mediates					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1375_s_135	7867176	38  Furthermore, oxidation of LDL, now thought to be a critical process in atherogenesis, 39  increases binding of LDL to collagen, 40  raising the possibility of damage to collagen or elastin fibers mediated by free radicals derived from lipid hydroperoxides and other reactive intermediaries.	bind
33411	8	7980	5	13	NULL	NULL	NULL	statement 5	Process		mediates					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1375_s_135	7867176	38  Furthermore, oxidation of LDL, now thought to be a critical process in atherogenesis, 39  increases binding of LDL to collagen, 40  raising the possibility of damage to collagen or elastin fibers mediated by free radicals derived from lipid hydroperoxides and other reactive intermediaries.	bind
33412	9	7980	5	13	NULL	NULL	NULL	statement 3	Process		damages		possibly			elastin fibers	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1375_s_135	7867176	38  Furthermore, oxidation of LDL, now thought to be a critical process in atherogenesis, 39  increases binding of LDL to collagen, 40  raising the possibility of damage to collagen or elastin fibers mediated by free radicals derived from lipid hydroperoxides and other reactive intermediaries.	bind
33413	10	7980	5	13	NULL	NULL	NULL	statement 4	Process		mediates					statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1375_s_135	7867176	38  Furthermore, oxidation of LDL, now thought to be a critical process in atherogenesis, 39  increases binding of LDL to collagen, 40  raising the possibility of damage to collagen or elastin fibers mediated by free radicals derived from lipid hydroperoxides and other reactive intermediaries.	bind
33414	11	7980	5	13	NULL	NULL	NULL	statement 5	Process		mediates					statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1375_s_135	7867176	38  Furthermore, oxidation of LDL, now thought to be a critical process in atherogenesis, 39  increases binding of LDL to collagen, 40  raising the possibility of damage to collagen or elastin fibers mediated by free radicals derived from lipid hydroperoxides and other reactive intermediaries.	bind
25874	1	7980	6	NULL	NULL	0	NULL	LDL	NULL	oxidation of	is a critical process in	NULL				atherogenesis	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_91_5_1375_s_135	7867176	38  Furthermore, oxidation of LDL, now thought to be a critical process in atherogenesis, 39  increases binding of LDL to collagen, 40  raising the possibility of damage to collagen or elastin fibers mediated by free radicals derived from lipid hydroperoxides and other reactive intermediaries.	bind
25875	2	7980	6	NULL	NULL	0	NULL	LDL	NULL		bind	NULL				collagen	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_91_5_1375_s_135	7867176	38  Furthermore, oxidation of LDL, now thought to be a critical process in atherogenesis, 39  increases binding of LDL to collagen, 40  raising the possibility of damage to collagen or elastin fibers mediated by free radicals derived from lipid hydroperoxides and other reactive intermediaries.	bind
26261	3	7980	6	NULL	NULL	0	NULL	LDL	NULL		bind	NULL				collagen	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1375_s_135	7867176	38  Furthermore, oxidation of LDL, now thought to be a critical process in atherogenesis, 39  increases binding of LDL to collagen, 40  raising the possibility of damage to collagen or elastin fibers mediated by free radicals derived from lipid hydroperoxides and other reactive intermediaries.	bind
26262	4	7980	6	NULL	NULL	0	NULL	LDL	NULL	oxidation of	increases	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1375_s_135	7867176	38  Furthermore, oxidation of LDL, now thought to be a critical process in atherogenesis, 39  increases binding of LDL to collagen, 40  raising the possibility of damage to collagen or elastin fibers mediated by free radicals derived from lipid hydroperoxides and other reactive intermediaries.	bind
26263	5	7980	6	NULL	NULL	0	NULL	free radicles	NULL		derived from	NULL				lipid hydroperoxides	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1375_s_135	7867176	38  Furthermore, oxidation of LDL, now thought to be a critical process in atherogenesis, 39  increases binding of LDL to collagen, 40  raising the possibility of damage to collagen or elastin fibers mediated by free radicals derived from lipid hydroperoxides and other reactive intermediaries.	bind
26264	6	7980	6	NULL	NULL	0	NULL	free radicles	NULL		mediates	NULL				elastin fibres	NULL	damage to			NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1375_s_135	7867176	38  Furthermore, oxidation of LDL, now thought to be a critical process in atherogenesis, 39  increases binding of LDL to collagen, 40  raising the possibility of damage to collagen or elastin fibers mediated by free radicals derived from lipid hydroperoxides and other reactive intermediaries.	bind
26265	7	7980	6	NULL	NULL	0	NULL	free radicles	NULL		mediates	NULL				collagen fibres	NULL	damage to			NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1375_s_135	7867176	38  Furthermore, oxidation of LDL, now thought to be a critical process in atherogenesis, 39  increases binding of LDL to collagen, 40  raising the possibility of damage to collagen or elastin fibers mediated by free radicals derived from lipid hydroperoxides and other reactive intermediaries.	bind
26266	8	7980	6	NULL	NULL	0	NULL	LDL	NULL	oxidation of	increases	NULL				statement 6	NULL	possibility of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1375_s_135	7867176	38  Furthermore, oxidation of LDL, now thought to be a critical process in atherogenesis, 39  increases binding of LDL to collagen, 40  raising the possibility of damage to collagen or elastin fibers mediated by free radicals derived from lipid hydroperoxides and other reactive intermediaries.	bind
26267	9	7980	6	NULL	NULL	0	NULL	LDL	NULL	oxidation of	increases	NULL				statement 7	NULL	possibility of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_5_1375_s_135	7867176	38  Furthermore, oxidation of LDL, now thought to be a critical process in atherogenesis, 39  increases binding of LDL to collagen, 40  raising the possibility of damage to collagen or elastin fibers mediated by free radicals derived from lipid hydroperoxides and other reactive intermediaries.	bind
33415	1	7981	5	13	NULL	NULL	NULL	LDL	GP		bind					LDLr	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_5_1301_s_40	10807746	38  Methods to determine the abilities of anti-apoB mAbs to block the binding of LDL to the LDLr and to bind to LDL in LDL-LDLr complexes have been described previously.	bind
33416	2	7981	5	13	NULL	NULL	NULL	anti-apoB mAbs	GP		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_5_1301_s_40	10807746	38  Methods to determine the abilities of anti-apoB mAbs to block the binding of LDL to the LDLr and to bind to LDL in LDL-LDLr complexes have been described previously.	bind
33417	4	7981	5	13	NULL	NULL	NULL	anti-apoB mAbs	GP		bind					statement 3	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_5_1301_s_40	10807746	38  Methods to determine the abilities of anti-apoB mAbs to block the binding of LDL to the LDLr and to bind to LDL in LDL-LDLr complexes have been described previously.	bind
47835	3	7981	5	13	NULL	NULL	NULL	LDL	GP		complex with					LDLr	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_5_1301_s_40	10807746	38  Methods to determine the abilities of anti-apoB mAbs to block the binding of LDL to the LDLr and to bind to LDL in LDL-LDLr complexes have been described previously.	bind
25876	1	7981	6	NULL	NULL	0	NULL	LDL	NULL		bind	NULL				LDLr	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_5_1301_s_40	10807746	38  Methods to determine the abilities of anti-apoB mAbs to block the binding of LDL to the LDLr and to bind to LDL in LDL-LDLr complexes have been described previously.	bind
25877	2	7981	6	NULL	NULL	0	NULL	anti-apoB mAbs	NULL		block	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_5_1301_s_40	10807746	38  Methods to determine the abilities of anti-apoB mAbs to block the binding of LDL to the LDLr and to bind to LDL in LDL-LDLr complexes have been described previously.	bind
47836	3	7981	6	10	NULL	0	NULL	LDL	NULL		complex with	NULL				LDLr	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_5_1301_s_40	10807746	38  Methods to determine the abilities of anti-apoB mAbs to block the binding of LDL to the LDLr and to bind to LDL in LDL-LDLr complexes have been described previously.	bind
47837	4	7981	6	10	NULL	0	NULL	anti-apoB mAbs	NULL		bind	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_5_1301_s_40	10807746	38  Methods to determine the abilities of anti-apoB mAbs to block the binding of LDL to the LDLr and to bind to LDL in LDL-LDLr complexes have been described previously.	bind
33418	1	7982	5	13	NULL	NULL	NULL	EKLF	GP		is					erythroid-specific Kruppel factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_6_978_s_254	8635248	38  Miller and Bieker 39  have isolated an erythroid-specific Kruppel factor (EKLF), containing proline-rich domains and three zinc-finger structures that bear some similarities with those in the Kruppel family of transcription factors, as a protein binding to the CACC-box of beta-globin.	bind
33419	2	7982	5	13	NULL	NULL	NULL	EKLF	GP		similar to			proline-rich domains;;zinc-finger structures		Kruppel transcription factors family	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_6_978_s_254	8635248	38  Miller and Bieker 39  have isolated an erythroid-specific Kruppel factor (EKLF), containing proline-rich domains and three zinc-finger structures that bear some similarities with those in the Kruppel family of transcription factors, as a protein binding to the CACC-box of beta-globin.	bind
33420	3	7982	5	13	NULL	NULL	NULL	EKLF	GP		bind					beta-globin	GP			CACC-box	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_6_978_s_254	8635248	38  Miller and Bieker 39  have isolated an erythroid-specific Kruppel factor (EKLF), containing proline-rich domains and three zinc-finger structures that bear some similarities with those in the Kruppel family of transcription factors, as a protein binding to the CACC-box of beta-globin.	bind
26268	1	7982	6	NULL	NULL	0	NULL	EKLF	NULL		is	NULL				erythroid-specific Kruppel factor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_78_6_978_s_254	8635248	38  Miller and Bieker 39  have isolated an erythroid-specific Kruppel factor (EKLF), containing proline-rich domains and three zinc-finger structures that bear some similarities with those in the Kruppel family of transcription factors, as a protein binding to the CACC-box of beta-globin.	bind
26269	2	7982	6	NULL	NULL	0	NULL	EKLF	NULL		contains	NULL					NULL		proline-rich domains		NULL		0	NULL	NULL	NULL	gw60_circulationres_78_6_978_s_254	8635248	38  Miller and Bieker 39  have isolated an erythroid-specific Kruppel factor (EKLF), containing proline-rich domains and three zinc-finger structures that bear some similarities with those in the Kruppel family of transcription factors, as a protein binding to the CACC-box of beta-globin.	bind
26270	3	7982	6	NULL	NULL	0	NULL	EKLF	NULL		contains	NULL					NULL		zinc-finger structures		NULL		0	NULL	NULL	NULL	gw60_circulationres_78_6_978_s_254	8635248	38  Miller and Bieker 39  have isolated an erythroid-specific Kruppel factor (EKLF), containing proline-rich domains and three zinc-finger structures that bear some similarities with those in the Kruppel family of transcription factors, as a protein binding to the CACC-box of beta-globin.	bind
26271	4	7982	6	NULL	NULL	0	NULL	EKLF	NULL		bind	NULL				beta-globin	NULL			CACC box	NULL		0	NULL	NULL	NULL	gw60_circulationres_78_6_978_s_254	8635248	38  Miller and Bieker 39  have isolated an erythroid-specific Kruppel factor (EKLF), containing proline-rich domains and three zinc-finger structures that bear some similarities with those in the Kruppel family of transcription factors, as a protein binding to the CACC-box of beta-globin.	bind
26917	5	7982	6	NULL	NULL	0	NULL	statement 2	NULL		occurs simultaneously with	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_78_6_978_s_254	8635248	38  Miller and Bieker 39  have isolated an erythroid-specific Kruppel factor (EKLF), containing proline-rich domains and three zinc-finger structures that bear some similarities with those in the Kruppel family of transcription factors, as a protein binding to the CACC-box of beta-globin.	bind
47838	6	7982	6	10	NULL	0	NULL	EKLF	NULL		is similar to	NULL		proline-rich domains;;zinc-finger structures		Kruppel transcription factors family	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_78_6_978_s_254	8635248	38  Miller and Bieker 39  have isolated an erythroid-specific Kruppel factor (EKLF), containing proline-rich domains and three zinc-finger structures that bear some similarities with those in the Kruppel family of transcription factors, as a protein binding to the CACC-box of beta-globin.	bind
33421	1	7983	5	13	NULL	NULL	NULL	fibrinogen	GP		bind					GP IIb/IIa receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_15_1481_s_171	9576429	38  The results of the present study are comparable to these findings, because the binding of fibrinogen to the GP IIb/IIa receptor was inhibited in vitro and during NO inhalation in patients with ARDS.	bind
33422	2	7983	5	13	NULL	NULL	NULL	NO	Chemical	inhalation of	inhibits					statement 1	Process				NULL	in patients with ARDS	NULL	NULL	NULL	NULL	gw60_circulation_97_15_1481_s_171	9576429	38  The results of the present study are comparable to these findings, because the binding of fibrinogen to the GP IIb/IIa receptor was inhibited in vitro and during NO inhalation in patients with ARDS.	bind
33423	3	7983	5	13	NULL	NULL	NULL	statement 1	Process		undergoes					inhibition	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulation_97_15_1481_s_171	9576429	38  The results of the present study are comparable to these findings, because the binding of fibrinogen to the GP IIb/IIa receptor was inhibited in vitro and during NO inhalation in patients with ARDS.	bind
25878	1	7983	6	NULL	NULL	0	NULL	fibrinogen	NULL		bind	NULL				GP IIb/IIa receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_97_15_1481_s_171	9576429	38  The results of the present study are comparable to these findings, because the binding of fibrinogen to the GP IIb/IIa receptor was inhibited in vitro and during NO inhalation in patients with ARDS.	bind
25879	2	7983	6	NULL	NULL	0	NULL	NO	NULL	inhalation of	inhibits	NULL				statement 1	NULL				NULL	patients with ARDS	NULL	NULL	NULL	NULL	gw60_circulation_97_15_1481_s_171	9576429	38  The results of the present study are comparable to these findings, because the binding of fibrinogen to the GP IIb/IIa receptor was inhibited in vitro and during NO inhalation in patients with ARDS.	bind
37882	3	7983	6	NULL	NULL	0	NULL	statement 1	NULL		undergoes 	NULL				inhibition	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulation_97_15_1481_s_171	9576429	38  The results of the present study are comparable to these findings, because the binding of fibrinogen to the GP IIb/IIa receptor was inhibited in vitro and during NO inhalation in patients with ARDS.	bind
33427	1	7985	5	13	NULL	NULL	NULL	insulin	GP		activates					p21ras	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_7_1086_s_219	12117721	38 The mechanism leading to the activation of p21ras by insulin is thought to involve binding of the phosphotyrosine-binding domain of IRS-1 to tyrosine-phosphorylated IRbeta.	bind
33428	2	7985	5	13	NULL	NULL	NULL	IRS-1	GP		bind			phosphotyrosine-binding domain		IRbeta	GP	tyrosine-phosphorylated			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_7_1086_s_219	12117721	38 The mechanism leading to the activation of p21ras by insulin is thought to involve binding of the phosphotyrosine-binding domain of IRS-1 to tyrosine-phosphorylated IRbeta.	bind
33429	3	7985	5	13	NULL	NULL	NULL	statement 2	Process		leads to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_7_1086_s_219	12117721	38 The mechanism leading to the activation of p21ras by insulin is thought to involve binding of the phosphotyrosine-binding domain of IRS-1 to tyrosine-phosphorylated IRbeta.	bind
25960	1	7985	6	NULL	NULL	0	NULL	insulin	NULL		activates	NULL				p21ras	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_7_1086_s_219	12117721	38 The mechanism leading to the activation of p21ras by insulin is thought to involve binding of the phosphotyrosine-binding domain of IRS-1 to tyrosine-phosphorylated IRbeta.	bind
25961	2	7985	6	NULL	NULL	0	NULL	IRS-1	NULL		bind	NULL		phosphotyrosine-binding domain		IRbeta	NULL	phosphorylated	tyrosine		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_7_1086_s_219	12117721	38 The mechanism leading to the activation of p21ras by insulin is thought to involve binding of the phosphotyrosine-binding domain of IRS-1 to tyrosine-phosphorylated IRbeta.	bind
25962	3	7985	6	NULL	NULL	0	NULL	statement 1	NULL		occurs via	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_7_1086_s_219	12117721	38 The mechanism leading to the activation of p21ras by insulin is thought to involve binding of the phosphotyrosine-binding domain of IRS-1 to tyrosine-phosphorylated IRbeta.	bind
33430	1	7986	5	13	NULL	NULL	NULL	p16INK4a	GP		bind					Cdk4	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_2_661_s_195	11485924	38, 39 The second mutation detected (c.262G>A; E88K) maps to a site implicated in the binding of p16INK4a to Cdk4 and Cdk6 39  and thus likely results in a functional impairment of the protein.	bind
33431	2	7986	5	13	NULL	NULL	NULL	p16INK4a	GP		bind					Cdk6	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_2_661_s_195	11485924	38, 39 The second mutation detected (c.262G>A; E88K) maps to a site implicated in the binding of p16INK4a to Cdk4 and Cdk6 39  and thus likely results in a functional impairment of the protein.	bind
33432	3	7986	5	13	NULL	NULL	NULL	p16INK4a	GP	mutant	impairs			c.262G>A;;E88K		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_2_661_s_195	11485924	38, 39 The second mutation detected (c.262G>A; E88K) maps to a site implicated in the binding of p16INK4a to Cdk4 and Cdk6 39  and thus likely results in a functional impairment of the protein.	bind
33433	4	7986	5	13	NULL	NULL	NULL	p16INK4a	GP	mutant	impairs			c.262G>A;;E88K		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_2_661_s_195	11485924	38, 39 The second mutation detected (c.262G>A; E88K) maps to a site implicated in the binding of p16INK4a to Cdk4 and Cdk6 39  and thus likely results in a functional impairment of the protein.	bind
36173	5	7986	5	13	NULL	NULL	NULL	p16INK4a	GP	mutant	impairs			c.262G>A;;E88K		p16INK4a	GP	function of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_2_661_s_195	11485924	38, 39 The second mutation detected (c.262G>A; E88K) maps to a site implicated in the binding of p16INK4a to Cdk4 and Cdk6 39  and thus likely results in a functional impairment of the protein.	bind
25963	1	7986	6	NULL	NULL	0	NULL	p16INK4a	NULL		bind	NULL				Cdk4	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_2_661_s_195	11485924	38, 39 The second mutation detected (c.262G>A; E88K) maps to a site implicated in the binding of p16INK4a to Cdk4 and Cdk6 39  and thus likely results in a functional impairment of the protein.	bind
25964	2	7986	6	NULL	NULL	0	NULL	p16INK4a	NULL		bind	NULL				Cdk6	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_2_661_s_195	11485924	38, 39 The second mutation detected (c.262G>A; E88K) maps to a site implicated in the binding of p16INK4a to Cdk4 and Cdk6 39  and thus likely results in a functional impairment of the protein.	bind
25965	3	7986	6	NULL	NULL	0	NULL	p16INK4a	NULL	mutant	impairs	NULL		c.262G>A; E88K		p16INK4a	NULL	function of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_2_661_s_195	11485924	38, 39 The second mutation detected (c.262G>A; E88K) maps to a site implicated in the binding of p16INK4a to Cdk4 and Cdk6 39  and thus likely results in a functional impairment of the protein.	bind
25966	4	7986	6	NULL	NULL	0	NULL	p16INK4a	NULL	mutant	impairs	NULL		c.262G>A; E88K		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_2_661_s_195	11485924	38, 39 The second mutation detected (c.262G>A; E88K) maps to a site implicated in the binding of p16INK4a to Cdk4 and Cdk6 39  and thus likely results in a functional impairment of the protein.	bind
25967	5	7986	6	NULL	NULL	0	NULL	p16INK4a	NULL	mutant	impairs	NULL		c.262G>A; E88K		statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_2_661_s_195	11485924	38, 39 The second mutation detected (c.262G>A; E88K) maps to a site implicated in the binding of p16INK4a to Cdk4 and Cdk6 39  and thus likely results in a functional impairment of the protein.	bind
33434	2	7988	5	13	NULL	NULL	NULL	statement 1	NucleicAcid		acts as					transcriptional repressor	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_783_s_363	11160902	39       Grigoriev,M., Praseuth,D., Robin,P., Hemar,A., Saison-Behmoaras,T., Dautry-Varsat,A., Thuong,N.T., Helene,C. and Harel-Bellan,A. (1992) A triple helix-forming oligonucleotide - intercalator conjugate acts as a transcriptional repressor via inhibition of NF kappa B binding to interleukin-2 receptor alpha-regulatory sequence.	bind
33435	3	7988	5	13	NULL	NULL	NULL	NF kappa B	GP		bind					interleukin-2 receptor	GP			alpha-regulatory sequence	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_783_s_363	11160902	39       Grigoriev,M., Praseuth,D., Robin,P., Hemar,A., Saison-Behmoaras,T., Dautry-Varsat,A., Thuong,N.T., Helene,C. and Harel-Bellan,A. (1992) A triple helix-forming oligonucleotide - intercalator conjugate acts as a transcriptional repressor via inhibition of NF kappa B binding to interleukin-2 receptor alpha-regulatory sequence.	bind
33436	4	7988	5	13	NULL	NULL	NULL	statement 1	Process		inhibit					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_783_s_363	11160902	39       Grigoriev,M., Praseuth,D., Robin,P., Hemar,A., Saison-Behmoaras,T., Dautry-Varsat,A., Thuong,N.T., Helene,C. and Harel-Bellan,A. (1992) A triple helix-forming oligonucleotide - intercalator conjugate acts as a transcriptional repressor via inhibition of NF kappa B binding to interleukin-2 receptor alpha-regulatory sequence.	bind
47839	1	7988	5	13	NULL	NULL	NULL	oligonucleotide-intercalator conjugate	NucleicAcid		forms					triple helix	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_783_s_363	11160902	39       Grigoriev,M., Praseuth,D., Robin,P., Hemar,A., Saison-Behmoaras,T., Dautry-Varsat,A., Thuong,N.T., Helene,C. and Harel-Bellan,A. (1992) A triple helix-forming oligonucleotide - intercalator conjugate acts as a transcriptional repressor via inhibition of NF kappa B binding to interleukin-2 receptor alpha-regulatory sequence.	bind
47841	5	7988	5	13	NULL	NULL	NULL	statement 2	Process		occur via					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_783_s_363	11160902	39       Grigoriev,M., Praseuth,D., Robin,P., Hemar,A., Saison-Behmoaras,T., Dautry-Varsat,A., Thuong,N.T., Helene,C. and Harel-Bellan,A. (1992) A triple helix-forming oligonucleotide - intercalator conjugate acts as a transcriptional repressor via inhibition of NF kappa B binding to interleukin-2 receptor alpha-regulatory sequence.	bind
25968	1	7988	6	NULL	NULL	0	NULL	NF kappa B	NULL		bind	NULL				interleukin-2 receptor	NULL			alpha-regulatory sequence	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_783_s_363	11160902	39       Grigoriev,M., Praseuth,D., Robin,P., Hemar,A., Saison-Behmoaras,T., Dautry-Varsat,A., Thuong,N.T., Helene,C. and Harel-Bellan,A. (1992) A triple helix-forming oligonucleotide - intercalator conjugate acts as a transcriptional repressor via inhibition of NF kappa B binding to interleukin-2 receptor alpha-regulatory sequence.	bind
25969	3	7988	6	10	NULL	0	NULL	statement 2	NULL		acts as a	NULL				transcriptional repressor	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_783_s_363	11160902	39       Grigoriev,M., Praseuth,D., Robin,P., Hemar,A., Saison-Behmoaras,T., Dautry-Varsat,A., Thuong,N.T., Helene,C. and Harel-Bellan,A. (1992) A triple helix-forming oligonucleotide - intercalator conjugate acts as a transcriptional repressor via inhibition of NF kappa B binding to interleukin-2 receptor alpha-regulatory sequence.	bind
25970	4	7988	6	10	NULL	0	NULL	statement 2	NULL		inhibits	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_783_s_363	11160902	39       Grigoriev,M., Praseuth,D., Robin,P., Hemar,A., Saison-Behmoaras,T., Dautry-Varsat,A., Thuong,N.T., Helene,C. and Harel-Bellan,A. (1992) A triple helix-forming oligonucleotide - intercalator conjugate acts as a transcriptional repressor via inhibition of NF kappa B binding to interleukin-2 receptor alpha-regulatory sequence.	bind
37402	5	7988	6	10	NULL	0	NULL	statement 3	NULL		occurs via	NULL				statement 4	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_783_s_363	11160902	39       Grigoriev,M., Praseuth,D., Robin,P., Hemar,A., Saison-Behmoaras,T., Dautry-Varsat,A., Thuong,N.T., Helene,C. and Harel-Bellan,A. (1992) A triple helix-forming oligonucleotide - intercalator conjugate acts as a transcriptional repressor via inhibition of NF kappa B binding to interleukin-2 receptor alpha-regulatory sequence.	bind
47840	2	7988	6	10	NULL	0	NULL	oligonucleotide-intercalator conjugate	NULL		forms	NULL				triple helix	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_783_s_363	11160902	39       Grigoriev,M., Praseuth,D., Robin,P., Hemar,A., Saison-Behmoaras,T., Dautry-Varsat,A., Thuong,N.T., Helene,C. and Harel-Bellan,A. (1992) A triple helix-forming oligonucleotide - intercalator conjugate acts as a transcriptional repressor via inhibition of NF kappa B binding to interleukin-2 receptor alpha-regulatory sequence.	bind
33437	1	7990	5	13	NULL	NULL	NULL	BBF-1	GP	binding activity of	is distinguishable from					MEF-2	GP	cardiac;;binding activity of			NULL	chicken embryos	NULL	NULL	NULL	NULL	gw60_circulationres_79_1_4_s_111	8925567	39  Analysis of chicken embryos revealed that binding activity of BBF-1 is distinguishable from cardiac MEF-2 and appears before that of MEF-2.	bind
33438	2	7990	5	13	NULL	NULL	NULL	BBF-1	GP	binding activity of	appears before					MEF-2	GP	binding activity of			NULL	chicken embryos	NULL	NULL	NULL	NULL	gw60_circulationres_79_1_4_s_111	8925567	39  Analysis of chicken embryos revealed that binding activity of BBF-1 is distinguishable from cardiac MEF-2 and appears before that of MEF-2.	bind
26272	1	7990	6	10	NULL	0	NULL	BBF-1	NULL	binding activity of	is distinguishable from	NULL				MEF-2	NULL	cardiac;; binding activity of			NULL	 chicken embryos	NULL	NULL	NULL	NULL	gw60_circulationres_79_1_4_s_111	8925567	39  Analysis of chicken embryos revealed that binding activity of BBF-1 is distinguishable from cardiac MEF-2 and appears before that of MEF-2.	bind
37403	2	7990	6	10	NULL	0	NULL	BBF-1		binding activity of	appears before					MEF-2		binding activity of			NULL	chicken embryos	NULL	NULL	NULL	NULL	gw60_circulationres_79_1_4_s_111	8925567	39  Analysis of chicken embryos revealed that binding activity of BBF-1 is distinguishable from cardiac MEF-2 and appears before that of MEF-2.	bind
33439	1	7991	5	13	NULL	NULL	NULL	tyrosine phosphatase beta	GP		is a type of					receptor protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_162_6_1857_s_22	12759243	39  In addition, the receptor protein tyrosine phosphatase beta present on glial tumor cells binds to FNIII A1, 2, and 4, suggesting it to be an adhesion receptor to ECM. 40  However, it is unclear whether the alternatively spliced region of Tn-C directly enhances progressive behavior of tumor cells.	bind
33440	2	7991	5	13	NULL	NULL	NULL	tyrosine phosphatase beta	GP		bind					FNIII A1	GP				NULL	glial tumor cells	NULL	NULL	NULL	NULL	gw60_amjpathol_162_6_1857_s_22	12759243	39  In addition, the receptor protein tyrosine phosphatase beta present on glial tumor cells binds to FNIII A1, 2, and 4, suggesting it to be an adhesion receptor to ECM. 40  However, it is unclear whether the alternatively spliced region of Tn-C directly enhances progressive behavior of tumor cells.	bind
33441	3	7991	5	13	NULL	NULL	NULL	tyrosine phosphatase beta	GP		bind					FNIII A2	GP				NULL	glial tumor cells	NULL	NULL	NULL	NULL	gw60_amjpathol_162_6_1857_s_22	12759243	39  In addition, the receptor protein tyrosine phosphatase beta present on glial tumor cells binds to FNIII A1, 2, and 4, suggesting it to be an adhesion receptor to ECM. 40  However, it is unclear whether the alternatively spliced region of Tn-C directly enhances progressive behavior of tumor cells.	bind
33442	4	7991	5	13	NULL	NULL	NULL	tyrosine phosphatase beta	GP		bind					FNIII A4	GP				NULL	glial tumor cells	NULL	NULL	NULL	NULL	gw60_amjpathol_162_6_1857_s_22	12759243	39  In addition, the receptor protein tyrosine phosphatase beta present on glial tumor cells binds to FNIII A1, 2, and 4, suggesting it to be an adhesion receptor to ECM. 40  However, it is unclear whether the alternatively spliced region of Tn-C directly enhances progressive behavior of tumor cells.	bind
33443	5	7991	5	13	NULL	NULL	NULL	tyrosine phosphatase beta	GP		adhere to					ECM	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_162_6_1857_s_22	12759243	39  In addition, the receptor protein tyrosine phosphatase beta present on glial tumor cells binds to FNIII A1, 2, and 4, suggesting it to be an adhesion receptor to ECM. 40  However, it is unclear whether the alternatively spliced region of Tn-C directly enhances progressive behavior of tumor cells.	bind
33444	6	7991	5	13	NULL	NULL	NULL	statement 2	Process		suggests					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_162_6_1857_s_22	12759243	39  In addition, the receptor protein tyrosine phosphatase beta present on glial tumor cells binds to FNIII A1, 2, and 4, suggesting it to be an adhesion receptor to ECM. 40  However, it is unclear whether the alternatively spliced region of Tn-C directly enhances progressive behavior of tumor cells.	bind
33445	7	7991	5	13	NULL	NULL	NULL	statement 3	Process		suggests					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_162_6_1857_s_22	12759243	39  In addition, the receptor protein tyrosine phosphatase beta present on glial tumor cells binds to FNIII A1, 2, and 4, suggesting it to be an adhesion receptor to ECM. 40  However, it is unclear whether the alternatively spliced region of Tn-C directly enhances progressive behavior of tumor cells.	bind
33446	8	7991	5	13	NULL	NULL	NULL	statement 4	Process		suggests					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_162_6_1857_s_22	12759243	39  In addition, the receptor protein tyrosine phosphatase beta present on glial tumor cells binds to FNIII A1, 2, and 4, suggesting it to be an adhesion receptor to ECM. 40  However, it is unclear whether the alternatively spliced region of Tn-C directly enhances progressive behavior of tumor cells.	bind
25971	1	7991	6	NULL	NULL	0	NULL	tyrosine phosphatase beta receptor protein	NULL		is present on	NULL				glial tumor cells	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_162_6_1857_s_22	12759243	39  In addition, the receptor protein tyrosine phosphatase beta present on glial tumor cells binds to FNIII A1, 2, and 4, suggesting it to be an adhesion receptor to ECM. 40  However, it is unclear whether the alternatively spliced region of Tn-C directly enhances progressive behavior of tumor cells.	bind
25982	2	7991	6	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL				FNIII A1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_162_6_1857_s_22	12759243	39  In addition, the receptor protein tyrosine phosphatase beta present on glial tumor cells binds to FNIII A1, 2, and 4, suggesting it to be an adhesion receptor to ECM. 40  However, it is unclear whether the alternatively spliced region of Tn-C directly enhances progressive behavior of tumor cells.	bind
25984	3	7991	6	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL				FNIII A2	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_162_6_1857_s_22	12759243	39  In addition, the receptor protein tyrosine phosphatase beta present on glial tumor cells binds to FNIII A1, 2, and 4, suggesting it to be an adhesion receptor to ECM. 40  However, it is unclear whether the alternatively spliced region of Tn-C directly enhances progressive behavior of tumor cells.	bind
25986	4	7991	6	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL				FNIII A4	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_162_6_1857_s_22	12759243	39  In addition, the receptor protein tyrosine phosphatase beta present on glial tumor cells binds to FNIII A1, 2, and 4, suggesting it to be an adhesion receptor to ECM. 40  However, it is unclear whether the alternatively spliced region of Tn-C directly enhances progressive behavior of tumor cells.	bind
25989	5	7991	6	NULL	NULL	0	NULL	tyrosine phosphatase beta	NULL		adhers to	NULL				ECM	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_162_6_1857_s_22	12759243	39  In addition, the receptor protein tyrosine phosphatase beta present on glial tumor cells binds to FNIII A1, 2, and 4, suggesting it to be an adhesion receptor to ECM. 40  However, it is unclear whether the alternatively spliced region of Tn-C directly enhances progressive behavior of tumor cells.	bind
47842	6	7991	6	10	NULL	0	NULL	statement 2	NULL		suggests	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_162_6_1857_s_22	12759243	39  In addition, the receptor protein tyrosine phosphatase beta present on glial tumor cells binds to FNIII A1, 2, and 4, suggesting it to be an adhesion receptor to ECM. 40  However, it is unclear whether the alternatively spliced region of Tn-C directly enhances progressive behavior of tumor cells.	bind
47844	7	7991	6	10	NULL	0	NULL	statement 3	NULL		suggests	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_162_6_1857_s_22	12759243	39  In addition, the receptor protein tyrosine phosphatase beta present on glial tumor cells binds to FNIII A1, 2, and 4, suggesting it to be an adhesion receptor to ECM. 40  However, it is unclear whether the alternatively spliced region of Tn-C directly enhances progressive behavior of tumor cells.	bind
47845	8	7991	6	10	NULL	0	NULL	statement 4	NULL		suggests	NULL				statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_162_6_1857_s_22	12759243	39  In addition, the receptor protein tyrosine phosphatase beta present on glial tumor cells binds to FNIII A1, 2, and 4, suggesting it to be an adhesion receptor to ECM. 40  However, it is unclear whether the alternatively spliced region of Tn-C directly enhances progressive behavior of tumor cells.	bind
33448	1	7992	5	13	NULL	NULL	NULL	130 kDa protein	GP	mouse	bind		tightly			calmodulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_1846_s_45	9351345	39  The cDNA encodes a protein of 130 kDa that in the mouse (and partially in humans) tightly binds calmodulin even when intracellular calcium levels are low.	bind
33449	2	7992	5	13	NULL	NULL	NULL	statement 1	Process		in presence of					intracellular calcium 	Chemical	low levels of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_1846_s_45	9351345	39  The cDNA encodes a protein of 130 kDa that in the mouse (and partially in humans) tightly binds calmodulin even when intracellular calcium levels are low.	bind
25991	1	7992	6	10	NULL	0	NULL	130 kDa protein	NULL	mouse	bind	NULL	tightly			calmodulin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_1846_s_45	9351345	39  The cDNA encodes a protein of 130 kDa that in the mouse (and partially in humans) tightly binds calmodulin even when intracellular calcium levels are low.	bind
25993	2	7992	6	NULL	NULL	0	NULL	statement 1	NULL		occurs in presence of	NULL				intracellular calcium 	NULL	low levels of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_1846_s_45	9351345	39  The cDNA encodes a protein of 130 kDa that in the mouse (and partially in humans) tightly binds calmodulin even when intracellular calcium levels are low.	bind
33450	1	7993	5	13	NULL	NULL	NULL	MMP-2	GP		bind					MT-MMP	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_1_82_s_207	null	39 42  MMP-2 binds MT-MMP and becomes activated possibly through its limited proteolysis by MT - MMP-1.	bind
33451	2	7993	5	13	NULL	NULL	NULL	MMP-2	GP		is proteolysed by					MT - MMP-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_1_82_s_207	null	39 42  MMP-2 binds MT-MMP and becomes activated possibly through its limited proteolysis by MT - MMP-1.	bind
33452	3	7993	5	13	NULL	NULL	NULL	statement 2	Process		activates					MMP-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_1_82_s_207	null	39 42  MMP-2 binds MT-MMP and becomes activated possibly through its limited proteolysis by MT - MMP-1.	bind
26004	1	7993	6	NULL	NULL	0	NULL	MMP-2	NULL		bind	NULL				MT-MMP	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_97_1_82_s_207	null	39 42  MMP-2 binds MT-MMP and becomes activated possibly through its limited proteolysis by MT - MMP-1.	bind
26005	3	7993	6	10	NULL	0	NULL	statement 2			activates					MMP-2					NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_1_82_s_207	null	39 42  MMP-2 binds MT-MMP and becomes activated possibly through its limited proteolysis by MT - MMP-1.	bind
26006	2	7993	6	10	NULL	0	NULL	MT-MMP-1			proteolyse					MMP-2					NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_1_82_s_207	null	39 42  MMP-2 binds MT-MMP and becomes activated possibly through its limited proteolysis by MT - MMP-1.	bind
33453	1	7994	5	13	NULL	NULL	NULL	IRS-1	GP		is dissociated from					PI3-K	GP		p85 subunit		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1142_s_171	15802620	39,40  In other cell types, phosphorylation of Ser612 and Ser302 are involved in dissociation of IRS-1 from the p85 subunit of PI3-K, whereas Ser307 phosphorylation inhibits the binding of IRS-1 to the insulin receptor and triggers IRS-1 degradation.	bind
33454	2	7994	5	13	NULL	NULL	NULL			phosphorylation of	is involved in			Ser612		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1142_s_171	15802620	39,40  In other cell types, phosphorylation of Ser612 and Ser302 are involved in dissociation of IRS-1 from the p85 subunit of PI3-K, whereas Ser307 phosphorylation inhibits the binding of IRS-1 to the insulin receptor and triggers IRS-1 degradation.	bind
33455	3	7994	5	13	NULL	NULL	NULL	IRS-1	GP		bind					insulin receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1142_s_171	15802620	39,40  In other cell types, phosphorylation of Ser612 and Ser302 are involved in dissociation of IRS-1 from the p85 subunit of PI3-K, whereas Ser307 phosphorylation inhibits the binding of IRS-1 to the insulin receptor and triggers IRS-1 degradation.	bind
33456	4	7994	5	13	NULL	NULL	NULL			phosphorylation of	inhibits			Ser307		statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1142_s_171	15802620	39,40  In other cell types, phosphorylation of Ser612 and Ser302 are involved in dissociation of IRS-1 from the p85 subunit of PI3-K, whereas Ser307 phosphorylation inhibits the binding of IRS-1 to the insulin receptor and triggers IRS-1 degradation.	bind
33457	5	7994	5	13	NULL	NULL	NULL	statement 4	Process		triggers					IRS-1	GP	degradation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1142_s_171	15802620	39,40  In other cell types, phosphorylation of Ser612 and Ser302 are involved in dissociation of IRS-1 from the p85 subunit of PI3-K, whereas Ser307 phosphorylation inhibits the binding of IRS-1 to the insulin receptor and triggers IRS-1 degradation.	bind
55575	6	7994	5	13	NULL	NULL	NULL			phosphorylation of	is involved in			Ser302		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1142_s_171	15802620	39,40  In other cell types, phosphorylation of Ser612 and Ser302 are involved in dissociation of IRS-1 from the p85 subunit of PI3-K, whereas Ser307 phosphorylation inhibits the binding of IRS-1 to the insulin receptor and triggers IRS-1 degradation.	bind
26007	1	7994	6	NULL	NULL	0	NULL	IRS-1	NULL		bind	NULL				insulin receptor	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1142_s_171	15802620	39,40  In other cell types, phosphorylation of Ser612 and Ser302 are involved in dissociation of IRS-1 from the p85 subunit of PI3-K, whereas Ser307 phosphorylation inhibits the binding of IRS-1 to the insulin receptor and triggers IRS-1 degradation.	bind
26273	2	7994	6	NULL	NULL	0	NULL		NULL	phosphorylation of	inhibits	NULL		Ser307		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1142_s_171	15802620	39,40  In other cell types, phosphorylation of Ser612 and Ser302 are involved in dissociation of IRS-1 from the p85 subunit of PI3-K, whereas Ser307 phosphorylation inhibits the binding of IRS-1 to the insulin receptor and triggers IRS-1 degradation.	bind
26274	3	7994	6	NULL	NULL	0	NULL		NULL	phosphorylation of	triggers	NULL		Ser307		IRS-1	NULL	degradation of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1142_s_171	15802620	39,40  In other cell types, phosphorylation of Ser612 and Ser302 are involved in dissociation of IRS-1 from the p85 subunit of PI3-K, whereas Ser307 phosphorylation inhibits the binding of IRS-1 to the insulin receptor and triggers IRS-1 degradation.	bind
26275	4	7994	6	10	NULL	0	NULL	IRS-1			dissociates from					PI3-K			p85 subunit		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1142_s_171	15802620	39,40  In other cell types, phosphorylation of Ser612 and Ser302 are involved in dissociation of IRS-1 from the p85 subunit of PI3-K, whereas Ser307 phosphorylation inhibits the binding of IRS-1 to the insulin receptor and triggers IRS-1 degradation.	bind
26276	5	7994	6	NULL	NULL	0	NULL		NULL	phosphorylation of	is involved in	NULL		Ser612		statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1142_s_171	15802620	39,40  In other cell types, phosphorylation of Ser612 and Ser302 are involved in dissociation of IRS-1 from the p85 subunit of PI3-K, whereas Ser307 phosphorylation inhibits the binding of IRS-1 to the insulin receptor and triggers IRS-1 degradation.	bind
26277	6	7994	6	NULL	NULL	0	NULL		NULL	phosphorylation of	is involved in	NULL		Ser302		statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1142_s_171	15802620	39,40  In other cell types, phosphorylation of Ser612 and Ser302 are involved in dissociation of IRS-1 from the p85 subunit of PI3-K, whereas Ser307 phosphorylation inhibits the binding of IRS-1 to the insulin receptor and triggers IRS-1 degradation.	bind
33458	1	7995	5	13	NULL	NULL	NULL	Rac1	GP		bind					p67 PHOX	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_730_s_84	16574914	39,40  The cardiovascular literature is, in contrast, replete with examinations of ROS-mediated effects that can be triggered, at least in part, by Rac1 binding to p67 PHOX, leading to activation of the NADPH oxidase system.	bind
33459	2	7995	5	13	NULL	NULL	NULL	ROS-mediated effects	Process		triggered by		partly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_730_s_84	16574914	39,40  The cardiovascular literature is, in contrast, replete with examinations of ROS-mediated effects that can be triggered, at least in part, by Rac1 binding to p67 PHOX, leading to activation of the NADPH oxidase system.	bind
33460	3	7995	5	13	NULL	NULL	NULL	statement 2	Process		leads to					NADPH oxidase system	Process	activation of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_730_s_84	16574914	39,40  The cardiovascular literature is, in contrast, replete with examinations of ROS-mediated effects that can be triggered, at least in part, by Rac1 binding to p67 PHOX, leading to activation of the NADPH oxidase system.	bind
26008	1	7995	6	NULL	NULL	0	NULL	Rac1	NULL		bind	NULL				p67 PHOX	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_6_730_s_84	16574914	39,40  The cardiovascular literature is, in contrast, replete with examinations of ROS-mediated effects that can be triggered, at least in part, by Rac1 binding to p67 PHOX, leading to activation of the NADPH oxidase system.	bind
26042	3	7995	6	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				NADPH oxidase system	NULL	activation of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_730_s_84	16574914	39,40  The cardiovascular literature is, in contrast, replete with examinations of ROS-mediated effects that can be triggered, at least in part, by Rac1 binding to p67 PHOX, leading to activation of the NADPH oxidase system.	bind
37404	2	7995	6	NULL	NULL	0	NULL	ROS-mediated effects	NULL		are triggered by	NULL	partly			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_730_s_84	16574914	39,40  The cardiovascular literature is, in contrast, replete with examinations of ROS-mediated effects that can be triggered, at least in part, by Rac1 binding to p67 PHOX, leading to activation of the NADPH oxidase system.	bind
33514	1	7996	5	13	NULL	NULL	NULL	ZO-1	GP		bind					occludin	GP		COOH-terminal cytoplasmic tail		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_62_s_162	16269664	39,43,45   Published evidence also indicates that binding of ZO-1 (and ZO-2/3) to the COOH-terminal cytoplasmic tail of occludin is important for targeting of the latter to the tight junction, as well as for its cytoskeletal tethering, 46 a process that is almost certainly sensitive to the phosphorylation state of the junctional and cytoskeletal components involved.	bind
33515	2	7996	5	13	NULL	NULL	NULL	ZO-2/3	GP		bind					occludin	GP		COOH-terminal cytoplasmic tail		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_62_s_162	16269664	39,43,45   Published evidence also indicates that binding of ZO-1 (and ZO-2/3) to the COOH-terminal cytoplasmic tail of occludin is important for targeting of the latter to the tight junction, as well as for its cytoskeletal tethering, 46 a process that is almost certainly sensitive to the phosphorylation state of the junctional and cytoskeletal components involved.	bind
33516	3	7996	5	13	NULL	NULL	NULL	occludin	GP		is targeted to					tight junction	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_62_s_162	16269664	39,43,45   Published evidence also indicates that binding of ZO-1 (and ZO-2/3) to the COOH-terminal cytoplasmic tail of occludin is important for targeting of the latter to the tight junction, as well as for its cytoskeletal tethering, 46 a process that is almost certainly sensitive to the phosphorylation state of the junctional and cytoskeletal components involved.	bind
33517	4	7996	5	13	NULL	NULL	NULL	occludin	GP		is tethered to					cytoskeleton	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_62_s_162	16269664	39,43,45   Published evidence also indicates that binding of ZO-1 (and ZO-2/3) to the COOH-terminal cytoplasmic tail of occludin is important for targeting of the latter to the tight junction, as well as for its cytoskeletal tethering, 46 a process that is almost certainly sensitive to the phosphorylation state of the junctional and cytoskeletal components involved.	bind
33518	5	7996	5	13	NULL	NULL	NULL	statement 1	Process		is important for					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_62_s_162	16269664	39,43,45   Published evidence also indicates that binding of ZO-1 (and ZO-2/3) to the COOH-terminal cytoplasmic tail of occludin is important for targeting of the latter to the tight junction, as well as for its cytoskeletal tethering, 46 a process that is almost certainly sensitive to the phosphorylation state of the junctional and cytoskeletal components involved.	bind
33519	6	7996	5	13	NULL	NULL	NULL	statement 1	Process		is important for					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_62_s_162	16269664	39,43,45   Published evidence also indicates that binding of ZO-1 (and ZO-2/3) to the COOH-terminal cytoplasmic tail of occludin is important for targeting of the latter to the tight junction, as well as for its cytoskeletal tethering, 46 a process that is almost certainly sensitive to the phosphorylation state of the junctional and cytoskeletal components involved.	bind
33520	7	7996	5	13	NULL	NULL	NULL	statement 2	Process		is important for					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_62_s_162	16269664	39,43,45   Published evidence also indicates that binding of ZO-1 (and ZO-2/3) to the COOH-terminal cytoplasmic tail of occludin is important for targeting of the latter to the tight junction, as well as for its cytoskeletal tethering, 46 a process that is almost certainly sensitive to the phosphorylation state of the junctional and cytoskeletal components involved.	bind
33521	8	7996	5	13	NULL	NULL	NULL	statement 2	Process		is important for					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_62_s_162	16269664	39,43,45   Published evidence also indicates that binding of ZO-1 (and ZO-2/3) to the COOH-terminal cytoplasmic tail of occludin is important for targeting of the latter to the tight junction, as well as for its cytoskeletal tethering, 46 a process that is almost certainly sensitive to the phosphorylation state of the junctional and cytoskeletal components involved.	bind
33522	9	7996	5	13	NULL	NULL	NULL	cytoskeletal tethering	Process		is sensitive to					junctional components	CellComponent	phosphorylation state of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_62_s_162	16269664	39,43,45   Published evidence also indicates that binding of ZO-1 (and ZO-2/3) to the COOH-terminal cytoplasmic tail of occludin is important for targeting of the latter to the tight junction, as well as for its cytoskeletal tethering, 46 a process that is almost certainly sensitive to the phosphorylation state of the junctional and cytoskeletal components involved.	bind
33523	10	7996	5	13	NULL	NULL	NULL	cytoskeletal tethering	Process		is sensitive to					cytoskeletal components	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_62_s_162	16269664	39,43,45   Published evidence also indicates that binding of ZO-1 (and ZO-2/3) to the COOH-terminal cytoplasmic tail of occludin is important for targeting of the latter to the tight junction, as well as for its cytoskeletal tethering, 46 a process that is almost certainly sensitive to the phosphorylation state of the junctional and cytoskeletal components involved.	bind
26043	1	7996	6	NULL	NULL	0	NULL	ZO-1	NULL		bind	NULL				occludin	NULL		COOH-terminal cytoplasmic tail 		NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_62_s_162	16269664	39,43,45   Published evidence also indicates that binding of ZO-1 (and ZO-2/3) to the COOH-terminal cytoplasmic tail of occludin is important for targeting of the latter to the tight junction, as well as for its cytoskeletal tethering, 46 a process that is almost certainly sensitive to the phosphorylation state of the junctional and cytoskeletal components involved.	bind
26044	2	7996	6	NULL	NULL	0	NULL	occludin	NULL		is targeted to	NULL				tight junction	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_62_s_162	16269664	39,43,45   Published evidence also indicates that binding of ZO-1 (and ZO-2/3) to the COOH-terminal cytoplasmic tail of occludin is important for targeting of the latter to the tight junction, as well as for its cytoskeletal tethering, 46 a process that is almost certainly sensitive to the phosphorylation state of the junctional and cytoskeletal components involved.	bind
26045	3	7996	6	NULL	NULL	0	NULL	statement 1	NULL		is important for	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_62_s_162	16269664	39,43,45   Published evidence also indicates that binding of ZO-1 (and ZO-2/3) to the COOH-terminal cytoplasmic tail of occludin is important for targeting of the latter to the tight junction, as well as for its cytoskeletal tethering, 46 a process that is almost certainly sensitive to the phosphorylation state of the junctional and cytoskeletal components involved.	bind
26046	4	7996	6	NULL	NULL	0	NULL	statement 1	NULL		is important for	NULL				occludin	NULL	cytoskeletal tethering of 			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_62_s_162	16269664	39,43,45   Published evidence also indicates that binding of ZO-1 (and ZO-2/3) to the COOH-terminal cytoplasmic tail of occludin is important for targeting of the latter to the tight junction, as well as for its cytoskeletal tethering, 46 a process that is almost certainly sensitive to the phosphorylation state of the junctional and cytoskeletal components involved.	bind
26047	5	7996	6	NULL	NULL	0	NULL	ZO-2/3	NULL		bind	NULL				occludin	NULL		COOH-terminal cytoplasmic tail		NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_62_s_162	16269664	39,43,45   Published evidence also indicates that binding of ZO-1 (and ZO-2/3) to the COOH-terminal cytoplasmic tail of occludin is important for targeting of the latter to the tight junction, as well as for its cytoskeletal tethering, 46 a process that is almost certainly sensitive to the phosphorylation state of the junctional and cytoskeletal components involved.	bind
26048	6	7996	6	NULL	NULL	0	NULL	statement 1	NULL		is sensitive to	NULL				junctional components	NULL	phosphorylation state of 			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_62_s_162	16269664	39,43,45   Published evidence also indicates that binding of ZO-1 (and ZO-2/3) to the COOH-terminal cytoplasmic tail of occludin is important for targeting of the latter to the tight junction, as well as for its cytoskeletal tethering, 46 a process that is almost certainly sensitive to the phosphorylation state of the junctional and cytoskeletal components involved.	bind
26050	7	7996	6	NULL	NULL	0	NULL	statement 1	NULL		is sensitive to	NULL				cytoskeletal components	NULL	phosphorylation state of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_62_s_162	16269664	39,43,45   Published evidence also indicates that binding of ZO-1 (and ZO-2/3) to the COOH-terminal cytoplasmic tail of occludin is important for targeting of the latter to the tight junction, as well as for its cytoskeletal tethering, 46 a process that is almost certainly sensitive to the phosphorylation state of the junctional and cytoskeletal components involved.	bind
33461	1	7997	5	13	NULL	NULL	NULL	Pten	GP		bind					p53	GP				NULL		NULL	NULL	NULL	NULL	gw60_cancercell_3_2_97_s_37	12620402	3: Pten binds to p53 resulting in increased p53 half-life.	bind
33462	2	7997	5	13	NULL	NULL	NULL	statement 1	Process		increase					p53	GP	half life of			NULL		NULL	NULL	NULL	NULL	gw60_cancercell_3_2_97_s_37	12620402	3: Pten binds to p53 resulting in increased p53 half-life.	bind
26052	1	7997	6	NULL	NULL	0	NULL	Pten	NULL		bind	NULL				p53	NULL				NULL		0	NULL	NULL	NULL	gw60_cancercell_3_2_97_s_37	12620402	3: Pten binds to p53 resulting in increased p53 half-life.	bind
26053	2	7997	6	NULL	NULL	0	NULL	statement 1	NULL		increases	NULL				p53	NULL	half life of			NULL		0	NULL	NULL	NULL	gw60_cancercell_3_2_97_s_37	12620402	3: Pten binds to p53 resulting in increased p53 half-life.	bind
33819	1	7998	5	13	NULL	NULL	NULL	3A9 cells	Cell		is specific for					 HEL	GP	epitope of	46-61		NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_3_1067_s_53	9448286	3A9 cells are specific for the epitope of residues 46-61 of hen egg lysozyme (46-61 HEL) ( 59), which associate in B cells with newly synthesized IAk molecules only when they are targeted to the loading compartment by Ii. 3B11 T cells recognize the epitope of residues 34-45 of HEL (34-45 HEL) that binds to recycling class II molecules ( 61).	bind
33820	2	7998	5	13	NULL	NULL	NULL	 46-61 HEL	GP		is					hen egg lysozyme	GP		residues 46-61 of		NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_3_1067_s_53	9448286	3A9 cells are specific for the epitope of residues 46-61 of hen egg lysozyme (46-61 HEL) ( 59), which associate in B cells with newly synthesized IAk molecules only when they are targeted to the loading compartment by Ii. 3B11 T cells recognize the epitope of residues 34-45 of HEL (34-45 HEL) that binds to recycling class II molecules ( 61).	bind
33822	3	7998	5	13	NULL	NULL	NULL	46-61 HEL	GP		associates with					IAk molecules	GP	newly synthesized			NULL	in B cells	NULL	NULL	NULL	NULL	gw60_pnas_95_3_1067_s_53	9448286	3A9 cells are specific for the epitope of residues 46-61 of hen egg lysozyme (46-61 HEL) ( 59), which associate in B cells with newly synthesized IAk molecules only when they are targeted to the loading compartment by Ii. 3B11 T cells recognize the epitope of residues 34-45 of HEL (34-45 HEL) that binds to recycling class II molecules ( 61).	bind
33823	4	7998	5	13	NULL	NULL	NULL	IAk molecules	GP	newly synthesized	is targeted to					loading compartment	CellComponent				NULL	in B cells	NULL	NULL	NULL	NULL	gw60_pnas_95_3_1067_s_53	9448286	3A9 cells are specific for the epitope of residues 46-61 of hen egg lysozyme (46-61 HEL) ( 59), which associate in B cells with newly synthesized IAk molecules only when they are targeted to the loading compartment by Ii. 3B11 T cells recognize the epitope of residues 34-45 of HEL (34-45 HEL) that binds to recycling class II molecules ( 61).	bind
33824	5	7998	5	13	NULL	NULL	NULL	Ii	GP		is required for					statement 4	Process				NULL	in B cells	NULL	NULL	NULL	NULL	gw60_pnas_95_3_1067_s_53	9448286	3A9 cells are specific for the epitope of residues 46-61 of hen egg lysozyme (46-61 HEL) ( 59), which associate in B cells with newly synthesized IAk molecules only when they are targeted to the loading compartment by Ii. 3B11 T cells recognize the epitope of residues 34-45 of HEL (34-45 HEL) that binds to recycling class II molecules ( 61).	bind
33825	6	7998	5	13	NULL	NULL	NULL	statement 3	Process		occurs following		only			statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_3_1067_s_53	9448286	3A9 cells are specific for the epitope of residues 46-61 of hen egg lysozyme (46-61 HEL) ( 59), which associate in B cells with newly synthesized IAk molecules only when they are targeted to the loading compartment by Ii. 3B11 T cells recognize the epitope of residues 34-45 of HEL (34-45 HEL) that binds to recycling class II molecules ( 61).	bind
33826	7	7998	5	13	NULL	NULL	NULL	34-45 HEL	GP		is					residues 34-45 of HEL	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_3_1067_s_53	9448286	3A9 cells are specific for the epitope of residues 46-61 of hen egg lysozyme (46-61 HEL) ( 59), which associate in B cells with newly synthesized IAk molecules only when they are targeted to the loading compartment by Ii. 3B11 T cells recognize the epitope of residues 34-45 of HEL (34-45 HEL) that binds to recycling class II molecules ( 61).	bind
33827	8	7998	5	13	NULL	NULL	NULL	3B11 T cells	Cell		recognize					34-45 HEL	GP	epitope of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_3_1067_s_53	9448286	3A9 cells are specific for the epitope of residues 46-61 of hen egg lysozyme (46-61 HEL) ( 59), which associate in B cells with newly synthesized IAk molecules only when they are targeted to the loading compartment by Ii. 3B11 T cells recognize the epitope of residues 34-45 of HEL (34-45 HEL) that binds to recycling class II molecules ( 61).	bind
33828	9	7998	5	13	NULL	NULL	NULL	34-45 HEL	GP		bind					class II molecules	GP	recycling			NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_3_1067_s_53	9448286	3A9 cells are specific for the epitope of residues 46-61 of hen egg lysozyme (46-61 HEL) ( 59), which associate in B cells with newly synthesized IAk molecules only when they are targeted to the loading compartment by Ii. 3B11 T cells recognize the epitope of residues 34-45 of HEL (34-45 HEL) that binds to recycling class II molecules ( 61).	bind
26278	1	7998	6	13	NULL	NULL	NULL	HEL	GP		is					hen egg lysozyme	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_3_1067_s_53	9448286	3A9 cells are specific for the epitope of residues 46-61 of hen egg lysozyme (46-61 HEL) ( 59), which associate in B cells with newly synthesized IAk molecules only when they are targeted to the loading compartment by Ii. 3B11 T cells recognize the epitope of residues 34-45 of HEL (34-45 HEL) that binds to recycling class II molecules ( 61).	bind
26279	2	7998	6	NULL	NULL	0	NULL	HEL	NULL		bind	NULL		residues 34-45		recycling class II molecules	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_3_1067_s_53	9448286	3A9 cells are specific for the epitope of residues 46-61 of hen egg lysozyme (46-61 HEL) ( 59), which associate in B cells with newly synthesized IAk molecules only when they are targeted to the loading compartment by Ii. 3B11 T cells recognize the epitope of residues 34-45 of HEL (34-45 HEL) that binds to recycling class II molecules ( 61).	bind
26280	3	7998	6	NULL	NULL	0	NULL	3B11 T cells	NULL		recognize	NULL				HEL	NULL		epitope of residues 34-45		NULL		0	NULL	NULL	NULL	gw60_pnas_95_3_1067_s_53	9448286	3A9 cells are specific for the epitope of residues 46-61 of hen egg lysozyme (46-61 HEL) ( 59), which associate in B cells with newly synthesized IAk molecules only when they are targeted to the loading compartment by Ii. 3B11 T cells recognize the epitope of residues 34-45 of HEL (34-45 HEL) that binds to recycling class II molecules ( 61).	bind
26281	4	7998	6	NULL	NULL	0	NULL	3A9 cells	NULL		recognize	NULL				HEL	NULL		epitope of residues 46-61		NULL		0	NULL	NULL	NULL	gw60_pnas_95_3_1067_s_53	9448286	3A9 cells are specific for the epitope of residues 46-61 of hen egg lysozyme (46-61 HEL) ( 59), which associate in B cells with newly synthesized IAk molecules only when they are targeted to the loading compartment by Ii. 3B11 T cells recognize the epitope of residues 34-45 of HEL (34-45 HEL) that binds to recycling class II molecules ( 61).	bind
26282	5	7998	6	NULL	NULL	0	NULL	HEL	NULL		associate with	NULL		epitope of residues 46-61		IAk molecules	NULL	newly synthesized			NULL	B cells	NULL	NULL	NULL	NULL	gw60_pnas_95_3_1067_s_53	9448286	3A9 cells are specific for the epitope of residues 46-61 of hen egg lysozyme (46-61 HEL) ( 59), which associate in B cells with newly synthesized IAk molecules only when they are targeted to the loading compartment by Ii. 3B11 T cells recognize the epitope of residues 34-45 of HEL (34-45 HEL) that binds to recycling class II molecules ( 61).	bind
26283	6	7998	6	10	NULL	0	NULL	IAk molecules	NULL	newly synthesized	are targeted to	NULL				loading compartment	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_3_1067_s_53	9448286	3A9 cells are specific for the epitope of residues 46-61 of hen egg lysozyme (46-61 HEL) ( 59), which associate in B cells with newly synthesized IAk molecules only when they are targeted to the loading compartment by Ii. 3B11 T cells recognize the epitope of residues 34-45 of HEL (34-45 HEL) that binds to recycling class II molecules ( 61).	bind
26284	7	7998	6	NULL	NULL	0	NULL	statement 6	NULL		occurs by	NULL				Ii	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_3_1067_s_53	9448286	3A9 cells are specific for the epitope of residues 46-61 of hen egg lysozyme (46-61 HEL) ( 59), which associate in B cells with newly synthesized IAk molecules only when they are targeted to the loading compartment by Ii. 3B11 T cells recognize the epitope of residues 34-45 of HEL (34-45 HEL) that binds to recycling class II molecules ( 61).	bind
26285	8	7998	6	NULL	NULL	0	NULL	statement 5	NULL		occurs in presence of	NULL	only			statement 6	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_3_1067_s_53	9448286	3A9 cells are specific for the epitope of residues 46-61 of hen egg lysozyme (46-61 HEL) ( 59), which associate in B cells with newly synthesized IAk molecules only when they are targeted to the loading compartment by Ii. 3B11 T cells recognize the epitope of residues 34-45 of HEL (34-45 HEL) that binds to recycling class II molecules ( 61).	bind
33538	1	7999	5	13	NULL	NULL	NULL	3Ac/Sub1 G-actin	GP		exchange					epsilonATP	Chemical	bound			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_40_29916_s_8	16882670	3Ac/Sub1 G-actin exchanged bound epsilonATP more slowly than wild type actin, and the exchange rate for 3Ac/Sub12 was even slower, similar to that for muscle actin.	bind
33539	2	7999	5	13	NULL	NULL	NULL	3Ac/Sub1 G-actin	GP		exchange					actin	GP	muscle			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_40_29916_s_8	16882670	3Ac/Sub1 G-actin exchanged bound epsilonATP more slowly than wild type actin, and the exchange rate for 3Ac/Sub12 was even slower, similar to that for muscle actin.	bind
33540	3	7999	5	13	NULL	NULL	NULL	statement 1	Process		slower than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_40_29916_s_8	16882670	3Ac/Sub1 G-actin exchanged bound epsilonATP more slowly than wild type actin, and the exchange rate for 3Ac/Sub12 was even slower, similar to that for muscle actin.	bind
33542	4	7999	5	13	NULL	NULL	NULL	3Ac/Sub12	GP	exchange rate for	is similar to					actin	GP	muscle			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_40_29916_s_8	16882670	3Ac/Sub1 G-actin exchanged bound epsilonATP more slowly than wild type actin, and the exchange rate for 3Ac/Sub12 was even slower, similar to that for muscle actin.	bind
26092	1	7999	6	10	NULL	0	NULL	3Ac/Sub1 G-actin	NULL		exchange	NULL				epsilonATP	NULL	bound			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_40_29916_s_8	16882670	3Ac/Sub1 G-actin exchanged bound epsilonATP more slowly than wild type actin, and the exchange rate for 3Ac/Sub12 was even slower, similar to that for muscle actin.	bind
26093	2	7999	6	10	NULL	0	NULL	3Ac/Sub1 G-actin	NULL		exchange	NULL				actin	NULL	wild type			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_40_29916_s_8	16882670	3Ac/Sub1 G-actin exchanged bound epsilonATP more slowly than wild type actin, and the exchange rate for 3Ac/Sub12 was even slower, similar to that for muscle actin.	bind
26094	3	7999	6	NULL	NULL	0	NULL	statement 1	NULL		is slower than	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_40_29916_s_8	16882670	3Ac/Sub1 G-actin exchanged bound epsilonATP more slowly than wild type actin, and the exchange rate for 3Ac/Sub12 was even slower, similar to that for muscle actin.	bind
37405	4	7999	6	10	NULL	0	NULL	3Ac/Sub12		exchange rate of 	is similar to					actin		muscle			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_40_29916_s_8	16882670	3Ac/Sub1 G-actin exchanged bound epsilonATP more slowly than wild type actin, and the exchange rate for 3Ac/Sub12 was even slower, similar to that for muscle actin.	bind
33544	1	8000	5	13	NULL	NULL	NULL	TAG	Chemical		is					6-aminomethyl-3-methyl-4H-1,2,4-benzothiadiazine 1,1-dioxide	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_6_1163_s_5	12684273	3Among the 19 structural analogues of taurine, 6-aminomethyl-3-methyl4HH1,2,4-benzothiadiazine 1,1-dioxide (TAG), 2-aminoethylarsonic (AEA), 2-hydroxyethanesulfonic (ISE) and ( plus-or-minus ) cis-2-aminocyclohexane sulfonic acids (CAHS) displaced [3]taurine binding ( Ki=0.13, 0.13, 13.5 and 4.0  muM, respectively).	bind
33546	2	8000	5	13	NULL	NULL	NULL	TAG	Chemical		displaces					[3H]taurine	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_6_1163_s_5	12684273	3Among the 19 structural analogues of taurine, 6-aminomethyl-3-methyl4HH1,2,4-benzothiadiazine 1,1-dioxide (TAG), 2-aminoethylarsonic (AEA), 2-hydroxyethanesulfonic (ISE) and ( plus-or-minus ) cis-2-aminocyclohexane sulfonic acids (CAHS) displaced [3]taurine binding ( Ki=0.13, 0.13, 13.5 and 4.0  muM, respectively).	bind
33548	3	8000	5	13	NULL	NULL	NULL	AEA	Chemical		is					2-aminoethylarsonic	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_6_1163_s_5	12684273	3Among the 19 structural analogues of taurine, 6-aminomethyl-3-methyl4HH1,2,4-benzothiadiazine 1,1-dioxide (TAG), 2-aminoethylarsonic (AEA), 2-hydroxyethanesulfonic (ISE) and ( plus-or-minus ) cis-2-aminocyclohexane sulfonic acids (CAHS) displaced [3]taurine binding ( Ki=0.13, 0.13, 13.5 and 4.0  muM, respectively).	bind
33551	4	8000	5	13	NULL	NULL	NULL	AEA	Chemical		displaces					[3H]taurine	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_6_1163_s_5	12684273	3Among the 19 structural analogues of taurine, 6-aminomethyl-3-methyl4HH1,2,4-benzothiadiazine 1,1-dioxide (TAG), 2-aminoethylarsonic (AEA), 2-hydroxyethanesulfonic (ISE) and ( plus-or-minus ) cis-2-aminocyclohexane sulfonic acids (CAHS) displaced [3]taurine binding ( Ki=0.13, 0.13, 13.5 and 4.0  muM, respectively).	bind
33552	5	8000	5	13	NULL	NULL	NULL	ISE	Chemical		is					2-hydroxyethanesulfonic	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_6_1163_s_5	12684273	3Among the 19 structural analogues of taurine, 6-aminomethyl-3-methyl4HH1,2,4-benzothiadiazine 1,1-dioxide (TAG), 2-aminoethylarsonic (AEA), 2-hydroxyethanesulfonic (ISE) and ( plus-or-minus ) cis-2-aminocyclohexane sulfonic acids (CAHS) displaced [3]taurine binding ( Ki=0.13, 0.13, 13.5 and 4.0  muM, respectively).	bind
33553	6	8000	5	13	NULL	NULL	NULL	ISE	Chemical		displaces					[3H]taurine	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_6_1163_s_5	12684273	3Among the 19 structural analogues of taurine, 6-aminomethyl-3-methyl4HH1,2,4-benzothiadiazine 1,1-dioxide (TAG), 2-aminoethylarsonic (AEA), 2-hydroxyethanesulfonic (ISE) and ( plus-or-minus ) cis-2-aminocyclohexane sulfonic acids (CAHS) displaced [3]taurine binding ( Ki=0.13, 0.13, 13.5 and 4.0  muM, respectively).	bind
33555	7	8000	5	13	NULL	NULL	NULL	CAHS	Chemical		is					( plus-or-minus ) cis-2-aminocyclohexane sulfonic acids	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_6_1163_s_5	12684273	3Among the 19 structural analogues of taurine, 6-aminomethyl-3-methyl4HH1,2,4-benzothiadiazine 1,1-dioxide (TAG), 2-aminoethylarsonic (AEA), 2-hydroxyethanesulfonic (ISE) and ( plus-or-minus ) cis-2-aminocyclohexane sulfonic acids (CAHS) displaced [3]taurine binding ( Ki=0.13, 0.13, 13.5 and 4.0  muM, respectively).	bind
33556	8	8000	5	13	NULL	NULL	NULL	CAHS	Chemical		displaces					[3H]taurine	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_6_1163_s_5	12684273	3Among the 19 structural analogues of taurine, 6-aminomethyl-3-methyl4HH1,2,4-benzothiadiazine 1,1-dioxide (TAG), 2-aminoethylarsonic (AEA), 2-hydroxyethanesulfonic (ISE) and ( plus-or-minus ) cis-2-aminocyclohexane sulfonic acids (CAHS) displaced [3]taurine binding ( Ki=0.13, 0.13, 13.5 and 4.0  muM, respectively).	bind
33558	9	8000	5	13	NULL	NULL	NULL	TAG	Chemical		is a structural analogue of					taurine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_6_1163_s_5	12684273	3Among the 19 structural analogues of taurine, 6-aminomethyl-3-methyl4HH1,2,4-benzothiadiazine 1,1-dioxide (TAG), 2-aminoethylarsonic (AEA), 2-hydroxyethanesulfonic (ISE) and ( plus-or-minus ) cis-2-aminocyclohexane sulfonic acids (CAHS) displaced [3]taurine binding ( Ki=0.13, 0.13, 13.5 and 4.0  muM, respectively).	bind
33559	10	8000	5	13	NULL	NULL	NULL	AEA	Chemical		is a structural analogue of					taurine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_6_1163_s_5	12684273	3Among the 19 structural analogues of taurine, 6-aminomethyl-3-methyl4HH1,2,4-benzothiadiazine 1,1-dioxide (TAG), 2-aminoethylarsonic (AEA), 2-hydroxyethanesulfonic (ISE) and ( plus-or-minus ) cis-2-aminocyclohexane sulfonic acids (CAHS) displaced [3]taurine binding ( Ki=0.13, 0.13, 13.5 and 4.0  muM, respectively).	bind
33561	11	8000	5	13	NULL	NULL	NULL	ISE	Chemical		is a structural analogue of					taurine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_6_1163_s_5	12684273	3Among the 19 structural analogues of taurine, 6-aminomethyl-3-methyl4HH1,2,4-benzothiadiazine 1,1-dioxide (TAG), 2-aminoethylarsonic (AEA), 2-hydroxyethanesulfonic (ISE) and ( plus-or-minus ) cis-2-aminocyclohexane sulfonic acids (CAHS) displaced [3]taurine binding ( Ki=0.13, 0.13, 13.5 and 4.0  muM, respectively).	bind
33562	12	8000	5	13	NULL	NULL	NULL	CAHS	Chemical		is structural analogue of					taurine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_6_1163_s_5	12684273	3Among the 19 structural analogues of taurine, 6-aminomethyl-3-methyl4HH1,2,4-benzothiadiazine 1,1-dioxide (TAG), 2-aminoethylarsonic (AEA), 2-hydroxyethanesulfonic (ISE) and ( plus-or-minus ) cis-2-aminocyclohexane sulfonic acids (CAHS) displaced [3]taurine binding ( Ki=0.13, 0.13, 13.5 and 4.0  muM, respectively).	bind
26095	1	8000	6	NULL	NULL	0	NULL	TAG	NULL		is	NULL				taurine, 6-aminomethyl-3-methyl4HH1,2,4-benzothiadiazine 1,1-dioxide 	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_138_6_1163_s_5	12684273	3Among the 19 structural analogues of taurine, 6-aminomethyl-3-methyl4HH1,2,4-benzothiadiazine 1,1-dioxide (TAG), 2-aminoethylarsonic (AEA), 2-hydroxyethanesulfonic (ISE) and ( plus-or-minus ) cis-2-aminocyclohexane sulfonic acids (CAHS) displaced [3]taurine binding ( Ki=0.13, 0.13, 13.5 and 4.0  muM, respectively).	bind
26098	2	8000	6	NULL	NULL	0	NULL	AEA	NULL		is	NULL				2-aminoethylarsonic	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_138_6_1163_s_5	12684273	3Among the 19 structural analogues of taurine, 6-aminomethyl-3-methyl4HH1,2,4-benzothiadiazine 1,1-dioxide (TAG), 2-aminoethylarsonic (AEA), 2-hydroxyethanesulfonic (ISE) and ( plus-or-minus ) cis-2-aminocyclohexane sulfonic acids (CAHS) displaced [3]taurine binding ( Ki=0.13, 0.13, 13.5 and 4.0  muM, respectively).	bind
26099	3	8000	6	NULL	NULL	0	NULL	ISE	NULL		is	NULL				2-hydroxyethanesulfonic	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_138_6_1163_s_5	12684273	3Among the 19 structural analogues of taurine, 6-aminomethyl-3-methyl4HH1,2,4-benzothiadiazine 1,1-dioxide (TAG), 2-aminoethylarsonic (AEA), 2-hydroxyethanesulfonic (ISE) and ( plus-or-minus ) cis-2-aminocyclohexane sulfonic acids (CAHS) displaced [3]taurine binding ( Ki=0.13, 0.13, 13.5 and 4.0  muM, respectively).	bind
26100	4	8000	6	NULL	NULL	0	NULL	CAHS	NULL		is	NULL				cis-2-aminocyclohexane sulfonic acids	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_138_6_1163_s_5	12684273	3Among the 19 structural analogues of taurine, 6-aminomethyl-3-methyl4HH1,2,4-benzothiadiazine 1,1-dioxide (TAG), 2-aminoethylarsonic (AEA), 2-hydroxyethanesulfonic (ISE) and ( plus-or-minus ) cis-2-aminocyclohexane sulfonic acids (CAHS) displaced [3]taurine binding ( Ki=0.13, 0.13, 13.5 and 4.0  muM, respectively).	bind
26101	5	8000	6	NULL	NULL	0	NULL	TAG	NULL		displaces	NULL				taurine	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_138_6_1163_s_5	12684273	3Among the 19 structural analogues of taurine, 6-aminomethyl-3-methyl4HH1,2,4-benzothiadiazine 1,1-dioxide (TAG), 2-aminoethylarsonic (AEA), 2-hydroxyethanesulfonic (ISE) and ( plus-or-minus ) cis-2-aminocyclohexane sulfonic acids (CAHS) displaced [3]taurine binding ( Ki=0.13, 0.13, 13.5 and 4.0  muM, respectively).	bind
26102	6	8000	6	NULL	NULL	0	NULL	AEA	NULL		displaces	NULL				taurine	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_138_6_1163_s_5	12684273	3Among the 19 structural analogues of taurine, 6-aminomethyl-3-methyl4HH1,2,4-benzothiadiazine 1,1-dioxide (TAG), 2-aminoethylarsonic (AEA), 2-hydroxyethanesulfonic (ISE) and ( plus-or-minus ) cis-2-aminocyclohexane sulfonic acids (CAHS) displaced [3]taurine binding ( Ki=0.13, 0.13, 13.5 and 4.0  muM, respectively).	bind
26105	7	8000	6	NULL	NULL	0	NULL	ISE	NULL		displaces	NULL				taurine	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_138_6_1163_s_5	12684273	3Among the 19 structural analogues of taurine, 6-aminomethyl-3-methyl4HH1,2,4-benzothiadiazine 1,1-dioxide (TAG), 2-aminoethylarsonic (AEA), 2-hydroxyethanesulfonic (ISE) and ( plus-or-minus ) cis-2-aminocyclohexane sulfonic acids (CAHS) displaced [3]taurine binding ( Ki=0.13, 0.13, 13.5 and 4.0  muM, respectively).	bind
26107	8	8000	6	NULL	NULL	0	NULL	CAHS	NULL		displaces	NULL				taurine	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_138_6_1163_s_5	12684273	3Among the 19 structural analogues of taurine, 6-aminomethyl-3-methyl4HH1,2,4-benzothiadiazine 1,1-dioxide (TAG), 2-aminoethylarsonic (AEA), 2-hydroxyethanesulfonic (ISE) and ( plus-or-minus ) cis-2-aminocyclohexane sulfonic acids (CAHS) displaced [3]taurine binding ( Ki=0.13, 0.13, 13.5 and 4.0  muM, respectively).	bind
37314	9	8000	6	10	NULL	0	NULL	TAG	NULL		is structural analogue of	NULL				 taurine	NULL				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_6_1163_s_5	12684273	3Among the 19 structural analogues of taurine, 6-aminomethyl-3-methyl4HH1,2,4-benzothiadiazine 1,1-dioxide (TAG), 2-aminoethylarsonic (AEA), 2-hydroxyethanesulfonic (ISE) and ( plus-or-minus ) cis-2-aminocyclohexane sulfonic acids (CAHS) displaced [3]taurine binding ( Ki=0.13, 0.13, 13.5 and 4.0  muM, respectively).	bind
37364	10	8000	6	10	NULL	0	NULL	AEA	NULL		is structural analogue of	NULL				 taurine	NULL				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_6_1163_s_5	12684273	3Among the 19 structural analogues of taurine, 6-aminomethyl-3-methyl4HH1,2,4-benzothiadiazine 1,1-dioxide (TAG), 2-aminoethylarsonic (AEA), 2-hydroxyethanesulfonic (ISE) and ( plus-or-minus ) cis-2-aminocyclohexane sulfonic acids (CAHS) displaced [3]taurine binding ( Ki=0.13, 0.13, 13.5 and 4.0  muM, respectively).	bind
37371	11	8000	6	10	NULL	0	NULL	ISE	NULL		is structural analogue of 	NULL				taurine	NULL				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_6_1163_s_5	12684273	3Among the 19 structural analogues of taurine, 6-aminomethyl-3-methyl4HH1,2,4-benzothiadiazine 1,1-dioxide (TAG), 2-aminoethylarsonic (AEA), 2-hydroxyethanesulfonic (ISE) and ( plus-or-minus ) cis-2-aminocyclohexane sulfonic acids (CAHS) displaced [3]taurine binding ( Ki=0.13, 0.13, 13.5 and 4.0  muM, respectively).	bind
37372	12	8000	6	10	NULL	0	NULL	CAHS	NULL		is structural analogue of	NULL				 taurine	NULL				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_6_1163_s_5	12684273	3Among the 19 structural analogues of taurine, 6-aminomethyl-3-methyl4HH1,2,4-benzothiadiazine 1,1-dioxide (TAG), 2-aminoethylarsonic (AEA), 2-hydroxyethanesulfonic (ISE) and ( plus-or-minus ) cis-2-aminocyclohexane sulfonic acids (CAHS) displaced [3]taurine binding ( Ki=0.13, 0.13, 13.5 and 4.0  muM, respectively).	bind
26108	1	8001	6	13	NULL	NULL	NULL	3beta,17betaAdiol	Chemical		is a type of					androgen metabolite	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_35_32086_s_68	12065592	3beta,17betaAdiol is a major androgen metabolite that binds human SHBG with high affinity ( 1).	bind
26109	2	8001	6	13	NULL	NULL	NULL	3beta,17betaAdiol	Chemical		bind		high affinity			SHBG	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_35_32086_s_68	12065592	3beta,17betaAdiol is a major androgen metabolite that binds human SHBG with high affinity ( 1).	bind
31329	1	8001	7	NULL	NULL	0	NULL	3beta,17betaAdiol	NULL		is a type of	NULL				androgen metabolite	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_35_32086_s_68	12065592	3beta,17betaAdiol is a major androgen metabolite that binds human SHBG with high affinity ( 1).	bind
31330	2	8001	7	NULL	NULL	0	NULL	3beta,17betaAdiol 	NULL		binds	NULL	high affinity			SHBG	NULL	human			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_35_32086_s_68	12065592	3beta,17betaAdiol is a major androgen metabolite that binds human SHBG with high affinity ( 1).	bind
26110	1	8002	6	13	NULL	NULL	NULL	3BP-1	GP		bind								SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_4_7_615_s_27	7953536	3BP-1 was found to bind to several different SH3 domains, but with significantly varying relative affinities.	bind
31331	1	8002	7	10	NULL	0	NULL	3BP-1 			bind								SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_4_7_615_s_27	7953536	3BP-1 was found to bind to several different SH3 domains, but with significantly varying relative affinities.	bind
26112	1	8003	6	13	NULL	NULL	NULL	3BP2	GP		bind					PTK c-Abl	GP		SH3 domain		NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_9_7146_s_22	12501243	3BP2 has been originally described as an  in vitro binding partner of the SH3 domain of the PTK c-Abl ( ).	bind
31332	1	8003	7	10	NULL	0	NULL	3BP2			bind					PTK c-Abl			SH3 domain		NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_9_7146_s_22	12501243	3BP2 has been originally described as an  in vitro binding partner of the SH3 domain of the PTK c-Abl ( ).	bind
26113	1	8007	6	13	NULL	NULL	NULL	MIB	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_1_155_s_118	9531555	3D map of MIB bound to actin.	bind
31333	1	8007	7	NULL	NULL	0	NULL	MIB	NULL		bind	NULL				actin	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_141_1_155_s_118	9531555	3D map of MIB bound to actin.	bind
26114	1	8008	6	13	NULL	NULL	NULL	ATP	Chemical		bind					CCT	GP				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_4_923_s_1976	10585970	3D reconstruction of the ATP-bound form of CCT reveals the asymetric folding conformation of a type II chaperonin.	bind
31334	1	8008	7	NULL	NULL	0	NULL	ATP	NULL		binds	NULL				CCT	NULL				NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_4_923_s_1976	10585970	3D reconstruction of the ATP-bound form of CCT reveals the asymetric folding conformation of a type II chaperonin.	bind
26117	1	8012	6	13	NULL	NULL	NULL	hRI	GP		bind					ANG	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_1_53_s_86	14681553	3D structures of hRI variants were modeled from the crystal structures of free pRI, pRI in its complex with RNase A, and hRI bound to human ANG [Protein Data Bank ID codes 1BNH [PDB] ( ), 1DFJ [PDB] ( ), and 1A4Y [PDB] ( ), respectively at the SWISS-MODEL server [ http://swissmodel.	bind
26118	2	8012	6	13	NULL	NULL	NULL	pRI	GP		forms a complex with					RNase A	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_1_53_s_86	14681553	3D structures of hRI variants were modeled from the crystal structures of free pRI, pRI in its complex with RNase A, and hRI bound to human ANG [Protein Data Bank ID codes 1BNH [PDB] ( ), 1DFJ [PDB] ( ), and 1A4Y [PDB] ( ), respectively at the SWISS-MODEL server [ http://swissmodel.	bind
31459	1	8012	7	NULL	NULL	0	NULL	pRI	NULL		complex with	NULL				RNase A	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_101_1_53_s_86	14681553	3D structures of hRI variants were modeled from the crystal structures of free pRI, pRI in its complex with RNase A, and hRI bound to human ANG [Protein Data Bank ID codes 1BNH [PDB] ( ), 1DFJ [PDB] ( ), and 1A4Y [PDB] ( ), respectively at the SWISS-MODEL server [ http://swissmodel.	bind
31460	2	8012	7	NULL	NULL	0	NULL	 hRI	NULL		bind	NULL				ANG	NULL	human			NULL		0	NULL	NULL	NULL	gw70_pnas_101_1_53_s_86	14681553	3D structures of hRI variants were modeled from the crystal structures of free pRI, pRI in its complex with RNase A, and hRI bound to human ANG [Protein Data Bank ID codes 1BNH [PDB] ( ), 1DFJ [PDB] ( ), and 1A4Y [PDB] ( ), respectively at the SWISS-MODEL server [ http://swissmodel.	bind
26119	1	8013	6	13	NULL	NULL	NULL	SfbI	GP		bind								NTD		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_37_39017_s_132	15247227	3F1 Is Involved in Binding of SfbI to the NTD --	bind
26120	2	8013	6	13	NULL	NULL	NULL	F1	GP		is involved in					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_37_39017_s_132	15247227	3F1 Is Involved in Binding of SfbI to the NTD --	bind
31461	1	8013	7	NULL	NULL	0	NULL	SfbI	NULL		bind	NULL					NULL		NTD		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_37_39017_s_132	15247227	3F1 Is Involved in Binding of SfbI to the NTD --	bind
31462	2	8013	7	NULL	NULL	0	NULL	F1	NULL		is involved in	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_37_39017_s_132	15247227	3F1 Is Involved in Binding of SfbI to the NTD --	bind
26122	1	8014	6	13	NULL	NULL	NULL	F10	GP		bind					SPN	GP	intracellular			NULL	rat pituitary cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_1_361_s_87	9417089	3F10 binding to intracellular SPN from rat pituitary cells is specifically blocked by preincubation of the mAb with pure native SPN ( 2).	bind
31463	1	8014	7	NULL	NULL	0	NULL	F10	NULL		bind	NULL				SPN	NULL	intracellular			NULL	rat pituitary cells	0	NULL	NULL	NULL	gw60_jbiolchem_273_1_361_s_87	9417089	3F10 binding to intracellular SPN from rat pituitary cells is specifically blocked by preincubation of the mAb with pure native SPN ( 2).	bind
26123	1	8016	6	13	NULL	NULL	NULL	3H Inhibitors	Chemical		does not bind					PDE5	GP	isolated	regulatory domain		NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_66_1_144_s_6	15213306	3H Inhibitors did not bind to isolated PDE5 regulatory domain.	bind
31465	1	8016	7	NULL	NULL	0	NULL	3H Inhibitors	NULL		does not bind	NULL				PDE5	NULL	isolated	regulatory domain		NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_66_1_144_s_6	15213306	3H Inhibitors did not bind to isolated PDE5 regulatory domain.	bind
46531	1	8018	6	13	NULL	NULL	NULL	3H-glutamate	Chemical		bind					NMDA receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_42_5_619_s_122	11985819	3H-glutamate binding to NMDA receptors	bind
31466	1	8018	7	NULL	NULL	0	NULL	3H-glutamate	NULL		bind	NULL				NMDA receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_42_5_619_s_122	11985819	3H-glutamate binding to NMDA receptors	bind
26124	1	8019	6	13	NULL	NULL	NULL	3H-heparin	Chemical		bind					whole Gc	Organism				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-exp-med_182_2_7629509_s_6	7629509	3H-heparin binding to whole Gc parallels  their adherence abilities (OpaA+ > OpaC+ > OpaH+ >> Opas B, D, E, F, G,  I = Opa- = 0).	bind
31467	1	8019	7	NULL	NULL	0	NULL	3H-heparin	NULL		bind	NULL				whole Gc	NULL				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_j-exp-med_182_2_7629509_s_6	7629509	3H-heparin binding to whole Gc parallels  their adherence abilities (OpaA+ > OpaC+ > OpaH+ >> Opas B, D, E, F, G,  I = Opa- = 0).	bind
26125	1	8020	6	13	NULL	NULL	NULL	3H-InsP3	Chemical		bind					InsP3R1	GP		NH2 terminus (aa 1-581)		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_2_312_s_299	14685260	3H-InsP3 binding to the NH2-terminal (aa 1 581) part of InsP3R1 (Lbs-1) was performed as described previously (  et al).	bind
46532	2	8020	6	13	NULL	NULL	NULL	InsP3R1	GP		is					Lbs-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_2_312_s_299	14685260	3H-InsP3 binding to the NH2-terminal (aa 1 581) part of InsP3R1 (Lbs-1) was performed as described previously (  et al).	bind
31469	1	8020	7	10	NULL	0	NULL	3H-InsP3			bind					 InsP3R1			NH2-terminal (aa-1581)		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_2_312_s_299	14685260	3H-InsP3 binding to the NH2-terminal (aa 1 581) part of InsP3R1 (Lbs-1) was performed as described previously (  et al).	bind
31470	2	8020	7	NULL	NULL	0	NULL	 InsP3R1	NULL		is	NULL				Lbs-1	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_23_2_312_s_299	14685260	3H-InsP3 binding to the NH2-terminal (aa 1 581) part of InsP3R1 (Lbs-1) was performed as described previously (  et al).	bind
26127	1	8021	6	13	NULL	NULL	NULL	kainate	Chemical		bind					hippocampus	OrganismPart				NULL	wild type mice	NULL	NULL	NULL	NULL	gw60_jneurosci_17_2_543_s_101	8987777	3H-kainate binding to the hippocampus in wild-type and  tPA /  mice	bind
26128	2	8021	6	13	NULL	NULL	NULL	kainate	Chemical		bind					hippocampus	OrganismPart				NULL	tPA mice	NULL	NULL	NULL	NULL	gw60_jneurosci_17_2_543_s_101	8987777	3H-kainate binding to the hippocampus in wild-type and  tPA /  mice	bind
31471	1	8021	7	NULL	NULL	0	NULL	3H-kainate	NULL		bind	NULL				hippocampus	NULL				NULL	wild-type mice	NULL	NULL	NULL	NULL	gw60_jneurosci_17_2_543_s_101	8987777	3H-kainate binding to the hippocampus in wild-type and  tPA /  mice	bind
31472	2	8021	7	NULL	NULL	0	NULL	3H-kainate	NULL		bind	NULL				hippocampus	NULL				NULL	tPA / mice	0	NULL	NULL	NULL	gw60_jneurosci_17_2_543_s_101	8987777	3H-kainate binding to the hippocampus in wild-type and  tPA /  mice	bind
26129	1	8024	6	13	NULL	NULL	NULL	GM1	Chemical	3H-labeled	bind					CD1b	GP	soluble			NULL		NULL	NULL	NULL	NULL	gw60_immunity_13_2_255_s_156	10981968	3H-labeled GM1 bound to soluble CD1b was displaced by cold GM2 (  Figure 5C).	bind
26130	2	8024	6	13	NULL	NULL	NULL	GM2	Chemical	cold	bind					CD1b	GP	soluble			NULL		NULL	NULL	NULL	NULL	gw60_immunity_13_2_255_s_156	10981968	3H-labeled GM1 bound to soluble CD1b was displaced by cold GM2 (  Figure 5C).	bind
55615	3	8024	6	13	NULL	NULL	NULL	statement 2	Process		displace					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_13_2_255_s_156	10981968	3H-labeled GM1 bound to soluble CD1b was displaced by cold GM2 (  Figure 5C).	bind
31473	1	8024	7	NULL	NULL	0	NULL	GM1	NULL	3H-labeled	bind	NULL				CD1b	NULL	soluble			NULL		0	NULL	NULL	NULL	gw60_immunity_13_2_255_s_156	10981968	3H-labeled GM1 bound to soluble CD1b was displaced by cold GM2 (  Figure 5C).	bind
31474	2	8024	7	10	NULL	0	NULL	GM2		cold	bind					CD1b		soluble			NULL		NULL	NULL	NULL	NULL	gw60_immunity_13_2_255_s_156	10981968	3H-labeled GM1 bound to soluble CD1b was displaced by cold GM2 (  Figure 5C).	bind
55804	3	8024	7	10	NULL	0	NULL	statement 2			displace					statement 1					NULL		0	NULL	NULL	NULL	gw60_immunity_13_2_255_s_156	10981968	3H-labeled GM1 bound to soluble CD1b was displaced by cold GM2 (  Figure 5C).	bind
26132	1	8026	6	13	NULL	NULL	NULL	prazosin	Chemical	3H-labeled	bind					cell membranes	CellComponent	fractionated			NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_286_2_984_s_87	9694959	3H-prazosin binding to fractionated cell membranes is the common method used to determine  alpha-1 adrenoceptor number and affinity (Kenny  et al., 1996  ).	bind
31475	1	8026	7	10	NULL	0	NULL	prazosin		3H labeled	bind					cell membranes		fractionated			NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_286_2_984_s_87	9694959	3H-prazosin binding to fractionated cell membranes is the common method used to determine  alpha-1 adrenoceptor number and affinity (Kenny  et al., 1996  ).	bind
26133	1	8027	6	13	NULL	NULL	NULL	reserpine	Chemical	3H-labeled	bind		irreversibly			transport protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevneurosci_20_0_125_s_152	9056710	3H-reserpine binds almost irreversibly to the transport protein, indicating that the  on-rate determines the affinity and providing a way to follow the protein during  purification ( Stern-Bach et al 1990).	bind
31477	1	8027	7	10	NULL	0	NULL	reserpine		3H-labeled	bind		irreversibly			transport protein					NULL		NULL	NULL	NULL	NULL	gw70_annurevneurosci_20_0_125_s_152	9056710	3H-reserpine binds almost irreversibly to the transport protein, indicating that the  on-rate determines the affinity and providing a way to follow the protein during  purification ( Stern-Bach et al 1990).	bind
26134	1	8028	6	13	NULL	NULL	NULL	RTX	Chemical	3H-labeled	bind							mutant	S512C		NULL		NULL	NULL	NULL	NULL	gw60_cell_108_3_421_s_162	11853675	3H-RTX bound to the S512C mutant with a KD of 310  plus-or-minus  20 pM (n = 2), only slightly higher than that of the wild-type receptor (200 pM).	bind
31478	1	8028	7	10	NULL	0	NULL	RTX 		3H-labeled \t	bind							mutant	S512C		NULL		NULL	NULL	NULL	NULL	gw60_cell_108_3_421_s_162	11853675	3H-RTX bound to the S512C mutant with a KD of 310  plus-or-minus  20 pM (n = 2), only slightly higher than that of the wild-type receptor (200 pM).	bind
26137	1	8029	6	13	NULL	NULL	NULL	SC52012B	Chemical	3H-labeled	bind					caspase-3	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_8_5760_s_244	10681563	3H-SC52012B bound to human caspase-3 to a greater extent than to a control milk protein.	bind
26765	2	8029	6	13	NULL	NULL	NULL	SC52012B	Chemical	3H-labeled	bind					milk protein	GP	control			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_8_5760_s_244	10681563	3H-SC52012B bound to human caspase-3 to a greater extent than to a control milk protein.	bind
26766	3	8029	6	13	NULL	NULL	NULL	statement 1	Process	affinity of	is greater than					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_8_5760_s_244	10681563	3H-SC52012B bound to human caspase-3 to a greater extent than to a control milk protein.	bind
31481	1	8029	7	10	NULL	0	NULL	SC52012B		3H-labeled	bind					caspase-3		human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_8_5760_s_244	10681563	3H-SC52012B bound to human caspase-3 to a greater extent than to a control milk protein.	bind
31482	2	8029	7	10	NULL	0	NULL	SC52012B		3H-labeled	bind					milk protein		control			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_8_5760_s_244	10681563	3H-SC52012B bound to human caspase-3 to a greater extent than to a control milk protein.	bind
31483	3	8029	7	NULL	NULL	0	NULL	statement 1	NULL	binding of	is greater than	NULL				statement 2	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_8_5760_s_244	10681563	3H-SC52012B bound to human caspase-3 to a greater extent than to a control milk protein.	bind
26136	1	8030	6	13	NULL	NULL	NULL	SC52012B	Chemical	3H-labeled	does not bind		specifically			milk protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_8_5760_s_188	10681563	3H-SC52012B showed no specific binding to 10% milk protein.	bind
31484	1	8030	7	10	NULL	0	NULL	SC52012B		3H-labeled	does not bind		specifically			milk protein					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_8_5760_s_188	10681563	3H-SC52012B showed no specific binding to 10% milk protein.	bind
26139	1	8031	6	13	NULL	NULL	NULL	SC52021B	Chemical	3H-labeled	bind					caspase-3	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_8_5760_s_178	10681563	3H-SC52021B binding to human caspase-3 (Fig.  5) was competed by unlabeled SC-52021B, orbofiban, xemilofiban, and by the monoclonal 7E3 antibody.	bind
26140	2	8031	6	13	NULL	NULL	NULL	SC-52021B	Chemical	unlabeled	bind					caspase-3	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_8_5760_s_178	10681563	3H-SC52021B binding to human caspase-3 (Fig.  5) was competed by unlabeled SC-52021B, orbofiban, xemilofiban, and by the monoclonal 7E3 antibody.	bind
26141	3	8031	6	13	NULL	NULL	NULL	statement 1	Process		competes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_8_5760_s_178	10681563	3H-SC52021B binding to human caspase-3 (Fig.  5) was competed by unlabeled SC-52021B, orbofiban, xemilofiban, and by the monoclonal 7E3 antibody.	bind
26142	4	8031	6	13	NULL	NULL	NULL	orbofiban	Chemical		bind					caspase-3	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_8_5760_s_178	10681563	3H-SC52021B binding to human caspase-3 (Fig.  5) was competed by unlabeled SC-52021B, orbofiban, xemilofiban, and by the monoclonal 7E3 antibody.	bind
26143	5	8031	6	13	NULL	NULL	NULL	statement 1	Process		competes					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_8_5760_s_178	10681563	3H-SC52021B binding to human caspase-3 (Fig.  5) was competed by unlabeled SC-52021B, orbofiban, xemilofiban, and by the monoclonal 7E3 antibody.	bind
26144	6	8031	6	13	NULL	NULL	NULL	xemilofiban	Chemical		bind					caspase-3	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_8_5760_s_178	10681563	3H-SC52021B binding to human caspase-3 (Fig.  5) was competed by unlabeled SC-52021B, orbofiban, xemilofiban, and by the monoclonal 7E3 antibody.	bind
26145	7	8031	6	13	NULL	NULL	NULL	statement 1	Process		competes					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_8_5760_s_178	10681563	3H-SC52021B binding to human caspase-3 (Fig.  5) was competed by unlabeled SC-52021B, orbofiban, xemilofiban, and by the monoclonal 7E3 antibody.	bind
26146	8	8031	6	13	NULL	NULL	NULL	monoclonal 7E3 antibody	GP		bind					caspase-3	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_8_5760_s_178	10681563	3H-SC52021B binding to human caspase-3 (Fig.  5) was competed by unlabeled SC-52021B, orbofiban, xemilofiban, and by the monoclonal 7E3 antibody.	bind
26147	9	8031	6	13	NULL	NULL	NULL	statement 1	Process		competes					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_8_5760_s_178	10681563	3H-SC52021B binding to human caspase-3 (Fig.  5) was competed by unlabeled SC-52021B, orbofiban, xemilofiban, and by the monoclonal 7E3 antibody.	bind
31493	1	8031	7	10	NULL	0	NULL	SC52021B		3H-labeled	bind					caspase-3		human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_8_5760_s_178	10681563	3H-SC52021B binding to human caspase-3 (Fig.  5) was competed by unlabeled SC-52021B, orbofiban, xemilofiban, and by the monoclonal 7E3 antibody.	bind
31494	2	8031	7	NULL	NULL	0	NULL	SC-52021B	NULL	unlabeled	bind	NULL				caspase-3	NULL	human			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_8_5760_s_178	10681563	3H-SC52021B binding to human caspase-3 (Fig.  5) was competed by unlabeled SC-52021B, orbofiban, xemilofiban, and by the monoclonal 7E3 antibody.	bind
31495	3	8031	7	NULL	NULL	0	NULL	orbofiban	NULL		bind	NULL				caspase-3	NULL	human			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_8_5760_s_178	10681563	3H-SC52021B binding to human caspase-3 (Fig.  5) was competed by unlabeled SC-52021B, orbofiban, xemilofiban, and by the monoclonal 7E3 antibody.	bind
31498	4	8031	7	NULL	NULL	0	NULL	xemilofiban	NULL		bind	NULL				caspase-3	NULL	human			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_8_5760_s_178	10681563	3H-SC52021B binding to human caspase-3 (Fig.  5) was competed by unlabeled SC-52021B, orbofiban, xemilofiban, and by the monoclonal 7E3 antibody.	bind
31500	5	8031	7	NULL	NULL	0	NULL	 monoclonal 7E3 antibody	NULL		bind	NULL				caspase-3	NULL	human			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_8_5760_s_178	10681563	3H-SC52021B binding to human caspase-3 (Fig.  5) was competed by unlabeled SC-52021B, orbofiban, xemilofiban, and by the monoclonal 7E3 antibody.	bind
31502	6	8031	7	NULL	NULL	0	NULL	statement 2	NULL		compete with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_8_5760_s_178	10681563	3H-SC52021B binding to human caspase-3 (Fig.  5) was competed by unlabeled SC-52021B, orbofiban, xemilofiban, and by the monoclonal 7E3 antibody.	bind
31503	7	8031	7	NULL	NULL	0	NULL	statement 3	NULL		compete with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_8_5760_s_178	10681563	3H-SC52021B binding to human caspase-3 (Fig.  5) was competed by unlabeled SC-52021B, orbofiban, xemilofiban, and by the monoclonal 7E3 antibody.	bind
31504	8	8031	7	NULL	NULL	0	NULL	statement 4	NULL		compete with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_8_5760_s_178	10681563	3H-SC52021B binding to human caspase-3 (Fig.  5) was competed by unlabeled SC-52021B, orbofiban, xemilofiban, and by the monoclonal 7E3 antibody.	bind
31505	9	8031	7	NULL	NULL	0	NULL	statement 5	NULL		compete with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_8_5760_s_178	10681563	3H-SC52021B binding to human caspase-3 (Fig.  5) was competed by unlabeled SC-52021B, orbofiban, xemilofiban, and by the monoclonal 7E3 antibody.	bind
26148	1	8032	6	13	NULL	NULL	NULL	SC52021B	Chemical	3H-labeled	bind					caspase-3	GP	recombinant;;human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_8_5760_s_177	10681563	3H-SC52021B Binding to Human Recombinant Caspase-3--3H-SC52021B bound to human recombinant caspase-3 with a  K d of 59  plus-or-minus  2 nM and a  Bmax of 324  plus-or-minus  32 fmol/mug of protein, ( n = 3).	bind
31511	1	8032	7	10	NULL	0	NULL	SC52021B		3H-labeled	bind					Caspase-3		human;;recombinant			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_8_5760_s_177	10681563	3H-SC52021B Binding to Human Recombinant Caspase-3--3H-SC52021B bound to human recombinant caspase-3 with a  K d of 59  plus-or-minus  2 nM and a  Bmax of 324  plus-or-minus  32 fmol/mug of protein, ( n = 3).	bind
26149	1	8035	6	13	NULL	NULL	NULL	LuxR	GP	purified	bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_3_631_s_82	14729687	3OC6-HSL-dependent DNA binding of purified LuxR.	bind
26150	2	8035	6	13	NULL	NULL	NULL	statement 1	Process		is dependent on					3OC6-HSL	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_3_631_s_82	14729687	3OC6-HSL-dependent DNA binding of purified LuxR.	bind
31512	1	8035	7	NULL	NULL	0	NULL	LuxR	NULL	purified	bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_3_631_s_82	14729687	3OC6-HSL-dependent DNA binding of purified LuxR.	bind
31513	2	8035	7	NULL	NULL	0	NULL	statement 1	NULL		depends on	NULL				3OC6-HSL	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_3_631_s_82	14729687	3OC6-HSL-dependent DNA binding of purified LuxR.	bind
26151	1	8037	6	13	NULL	NULL	NULL	3pK	GP		bind					E47	GP				NULL	in vivo in Yeast	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_27_20239_s_75	10781029	3pK Binds to E47 in Vivo in Yeast and Mammalian Cells-- To unravel the unknown physiological function of 3pK, we searched for binding partners in a yeast two-hybrid screen.	bind
46533	2	8037	6	13	NULL	NULL	NULL	3pK	GP		bind					E47	GP				NULL	in vivo in mammalian cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_27_20239_s_75	10781029	3pK Binds to E47 in Vivo in Yeast and Mammalian Cells-- To unravel the unknown physiological function of 3pK, we searched for binding partners in a yeast two-hybrid screen.	bind
31535	1	8037	7	NULL	NULL	0	NULL	3pK	NULL		binds to	NULL				 E47	NULL				NULL	in Vivo in Yeast 	0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20239_s_75	10781029	3pK Binds to E47 in Vivo in Yeast and Mammalian Cells-- To unravel the unknown physiological function of 3pK, we searched for binding partners in a yeast two-hybrid screen.	bind
31536	2	8037	7	NULL	NULL	0	NULL	3pK	NULL		binds to	NULL				E47	NULL				NULL	in vivo in mammalian cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_27_20239_s_75	10781029	3pK Binds to E47 in Vivo in Yeast and Mammalian Cells-- To unravel the unknown physiological function of 3pK, we searched for binding partners in a yeast two-hybrid screen.	bind
26152	1	8038	6	13	NULL	NULL	NULL	3R-tau	GP		bind					Fyn	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_42_35119_s_87	16115884	3R-tau Binds to Fyn SH3 with a Higher Affinity than 4R-tau --	bind
26153	2	8038	6	13	NULL	NULL	NULL	4R-tau	GP		bind					Fyn	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_42_35119_s_87	16115884	3R-tau Binds to Fyn SH3 with a Higher Affinity than 4R-tau --	bind
26154	3	8038	6	13	NULL	NULL	NULL	statement 1	Process	affinity of	is higher as compared to					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_42_35119_s_87	16115884	3R-tau Binds to Fyn SH3 with a Higher Affinity than 4R-tau --	bind
31537	1	8038	7	10	NULL	0	NULL	3R-tau			binds					Fyn			SH3		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_42_35119_s_87	16115884	3R-tau Binds to Fyn SH3 with a Higher Affinity than 4R-tau --	bind
31538	2	8038	7	NULL	NULL	0	NULL	4R-tau	NULL		binds	NULL				Fyn	NULL		SH3		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_42_35119_s_87	16115884	3R-tau Binds to Fyn SH3 with a Higher Affinity than 4R-tau --	bind
31539	3	8038	7	10	NULL	0	NULL	statement 1	NULL		higher affinity than	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_42_35119_s_87	16115884	3R-tau Binds to Fyn SH3 with a Higher Affinity than 4R-tau --	bind
31540	1	8039	7	13	NULL	NULL	NULL	3R-tau	GP		binds					GST-Fyn	GP		SH3		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_42_35119_s_109	16115884	3R-tau binds to GST-Fyn SH3 with a higher affinity than 4R-tau.	bind
31541	2	8039	7	13	NULL	NULL	NULL	4R-tau	GP		binds					GST-Fyn	GP		SH3		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_42_35119_s_109	16115884	3R-tau binds to GST-Fyn SH3 with a higher affinity than 4R-tau.	bind
31542	3	8039	7	13	NULL	NULL	NULL	statement 1	Process		higher affinity than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_42_35119_s_109	16115884	3R-tau binds to GST-Fyn SH3 with a higher affinity than 4R-tau.	bind
26155	1	8040	6	13	NULL	NULL	NULL	3T3 cells	Cell		express					ApoER2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_19_s_165	16354676	3T3 cells expressing ApoER2 or VLDLR bind Reelin.	bind
26156	2	8040	6	13	NULL	NULL	NULL	statement 1	GP		bind					Reelin	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_19_s_165	16354676	3T3 cells expressing ApoER2 or VLDLR bind Reelin.	bind
26157	3	8040	6	13	NULL	NULL	NULL	3T3 cells	Cell		express					VLDLR	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_19_s_165	16354676	3T3 cells expressing ApoER2 or VLDLR bind Reelin.	bind
26158	4	8040	6	13	NULL	NULL	NULL	statement 3	GP		bind					Reelin	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_19_s_165	16354676	3T3 cells expressing ApoER2 or VLDLR bind Reelin.	bind
26159	5	8040	6	13	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_19_s_165	16354676	3T3 cells expressing ApoER2 or VLDLR bind Reelin.	bind
31543	3	8040	7	10	NULL	0	NULL	statement 1	NULL		bind	NULL				Reelin	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_19_s_165	16354676	3T3 cells expressing ApoER2 or VLDLR bind Reelin.	bind
31544	4	8040	7	10	NULL	0	NULL	statement 3	NULL		bind	NULL				Reelin	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_1_19_s_165	16354676	3T3 cells expressing ApoER2 or VLDLR bind Reelin.	bind
46534	1	8040	7	10	NULL	0	NULL	3T3 cells	NULL		express	NULL				ApoER2	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_1_19_s_165	16354676	3T3 cells expressing ApoER2 or VLDLR bind Reelin.	bind
46535	2	8040	7	10	NULL	0	NULL	3T3 cells	NULL		express	NULL				VLDLR	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_1_19_s_165	16354676	3T3 cells expressing ApoER2 or VLDLR bind Reelin.	bind
46536	5	8040	7	10	NULL	0	NULL	statement 3	NULL		is an alternative to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_1_19_s_165	16354676	3T3 cells expressing ApoER2 or VLDLR bind Reelin.	bind
26160	1	8042	6	13	NULL	NULL	NULL	M4 oligonucleotide	NucleicAcid		bind					NF1 proteins	GP				NULL	3T3-L1 adipocyte nuclear extract	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_1712_s_191	11696544	3T3-L1 adipocyte nuclear extract was incubated with the  glut4-response element probe in the presence of increasing amounts of competitor M4 oligonucleotide which is bound by NF1 proteins but is not bound by O/E proteins.	bind
26161	2	8042	6	13	NULL	NULL	NULL	M4 oligonucleotide	NucleicAcid		does not bind					O/E proteins	GP				NULL	3T3-L1 adipocyte nuclear extract	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_1712_s_191	11696544	3T3-L1 adipocyte nuclear extract was incubated with the  glut4-response element probe in the presence of increasing amounts of competitor M4 oligonucleotide which is bound by NF1 proteins but is not bound by O/E proteins.	bind
31570	1	8042	7	NULL	NULL	0	NULL	NF1 proteins 	NULL		bind	NULL				M4 oligonucleotide	NULL				NULL	3T3-L1 adipocyte nuclear extract 	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_1712_s_191	11696544	3T3-L1 adipocyte nuclear extract was incubated with the  glut4-response element probe in the presence of increasing amounts of competitor M4 oligonucleotide which is bound by NF1 proteins but is not bound by O/E proteins.	bind
31571	2	8042	7	NULL	NULL	0	NULL	O/E proteins	NULL		does not bind	NULL				M4 oligonucleotide	NULL				NULL	3T3-L1 adipocyte nuclear extract 	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_1712_s_191	11696544	3T3-L1 adipocyte nuclear extract was incubated with the  glut4-response element probe in the presence of increasing amounts of competitor M4 oligonucleotide which is bound by NF1 proteins but is not bound by O/E proteins.	bind
26162	1	8043	6	13	NULL	NULL	NULL	spectrin	GP		does not bind			SH3 domain		dynamin	GP				NULL	3T3-L1 adipocytes	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_14_8169_s_176	9525921	3T3-L1 adipocytes were microinjected with fusion proteins containing the SH3 domains of spectrin and Crk (Fig.  5 A), which do not bind dynamin ( 23).	bind
26163	2	8043	6	13	NULL	NULL	NULL	Crk	GP		does not bind			SH3 domain		dynamin	GP				NULL	3T3-L1 adipocytes	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_14_8169_s_176	9525921	3T3-L1 adipocytes were microinjected with fusion proteins containing the SH3 domains of spectrin and Crk (Fig.  5 A), which do not bind dynamin ( 23).	bind
31574	1	8043	7	NULL	NULL	0	NULL	 spectrin	NULL		does not bind	NULL		SH3 domain		dynamin	NULL				NULL	3T3-L1 adipocytes 	0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8169_s_176	9525921	3T3-L1 adipocytes were microinjected with fusion proteins containing the SH3 domains of spectrin and Crk (Fig.  5 A), which do not bind dynamin ( 23).	bind
31576	2	8043	7	NULL	NULL	0	NULL	Crk	NULL		does not bind	NULL		SH3 domain		dynamin	NULL				NULL	3T3-L1 adipocytes	0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8169_s_176	9525921	3T3-L1 adipocytes were microinjected with fusion proteins containing the SH3 domains of spectrin and Crk (Fig.  5 A), which do not bind dynamin ( 23).	bind
26164	1	8044	6	13	NULL	NULL	NULL	AFP	GP	unlabeled	bind					MDM	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_3_507_s_40	12176010	3x105 cpm) binding to MDM by unlabeled AFP or MIP-1  were analyzed by fitting to a logistic curve or according to Scatchard.	bind
26165	2	8044	6	13	NULL	NULL	NULL	MIP-1	GP	unlabeled	bind					MDM	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_3_507_s_40	12176010	3x105 cpm) binding to MDM by unlabeled AFP or MIP-1  were analyzed by fitting to a logistic curve or according to Scatchard.	bind
31579	1	8044	7	NULL	NULL	0	NULL	AFP	NULL	unlabeled	bind	NULL				MDM	NULL				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_3_507_s_40	12176010	3x105 cpm) binding to MDM by unlabeled AFP or MIP-1  were analyzed by fitting to a logistic curve or according to Scatchard.	bind
31580	2	8044	7	NULL	NULL	0	NULL	MIP-1	NULL	unlabeled	bind	NULL				MDM	NULL				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_3_507_s_40	12176010	3x105 cpm) binding to MDM by unlabeled AFP or MIP-1  were analyzed by fitting to a logistic curve or according to Scatchard.	bind
26166	1	8046	6	13	NULL	NULL	NULL	Y-box binding protein 1	GP		bind		preferentially			DNA	NucleicAcid	cisplatin-modified			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_5_1200_s_259	11222770	4       Ise,T., Nagatani,G., Imamura,T., Kato,K., Takano,H., Nomoto,M., Izumi,H., Ohmori,H., Okamoto,T., Ohga,T., Uchiumi,T., Kuwano,M. and Kohno,K. (1999) Transcription factor Y-box binding protein 1 binds preferentially to cisplatin-modified DNA and interacts with proliferating cell nuclear antigen.	bind
26167	2	8046	6	13	NULL	NULL	NULL	Y-box binding protein 1	GP		interacts with					proliferating cell nuclear antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_5_1200_s_259	11222770	4       Ise,T., Nagatani,G., Imamura,T., Kato,K., Takano,H., Nomoto,M., Izumi,H., Ohmori,H., Okamoto,T., Ohga,T., Uchiumi,T., Kuwano,M. and Kohno,K. (1999) Transcription factor Y-box binding protein 1 binds preferentially to cisplatin-modified DNA and interacts with proliferating cell nuclear antigen.	bind
46537	3	8046	6	13	NULL	NULL	NULL	\tY-box binding protein 1 	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_5_1200_s_259	11222770	4       Ise,T., Nagatani,G., Imamura,T., Kato,K., Takano,H., Nomoto,M., Izumi,H., Ohmori,H., Okamoto,T., Ohga,T., Uchiumi,T., Kuwano,M. and Kohno,K. (1999) Transcription factor Y-box binding protein 1 binds preferentially to cisplatin-modified DNA and interacts with proliferating cell nuclear antigen.	bind
31583	1	8046	7	10	NULL	0	NULL	Y-box binding protein 1	NULL		binds	NULL	preferentially			DNA	NULL	 cisplatin-modified			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_5_1200_s_259	11222770	4       Ise,T., Nagatani,G., Imamura,T., Kato,K., Takano,H., Nomoto,M., Izumi,H., Ohmori,H., Okamoto,T., Ohga,T., Uchiumi,T., Kuwano,M. and Kohno,K. (1999) Transcription factor Y-box binding protein 1 binds preferentially to cisplatin-modified DNA and interacts with proliferating cell nuclear antigen.	bind
31584	2	8046	7	10	NULL	0	NULL	Y-box binding protein 1	NULL		interacts with	NULL				proliferating cell nuclear antigen	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_5_1200_s_259	11222770	4       Ise,T., Nagatani,G., Imamura,T., Kato,K., Takano,H., Nomoto,M., Izumi,H., Ohmori,H., Okamoto,T., Ohga,T., Uchiumi,T., Kuwano,M. and Kohno,K. (1999) Transcription factor Y-box binding protein 1 binds preferentially to cisplatin-modified DNA and interacts with proliferating cell nuclear antigen.	bind
46538	3	8046	7	10	NULL	0	NULL	Y-box binding protein 1	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_5_1200_s_259	11222770	4       Ise,T., Nagatani,G., Imamura,T., Kato,K., Takano,H., Nomoto,M., Izumi,H., Ohmori,H., Okamoto,T., Ohga,T., Uchiumi,T., Kuwano,M. and Kohno,K. (1999) Transcription factor Y-box binding protein 1 binds preferentially to cisplatin-modified DNA and interacts with proliferating cell nuclear antigen.	bind
26168	1	8047	6	13	NULL	NULL	NULL	uterine estrogen receptor	GP	purified;;calf	bind		high affinity			DNA	NucleicAcid			estrogen response element	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_219	11452016	4       Klinge,C.M., Brolly,C.L., Bambara,R.A. and Hilf,R. (1997) Hsp70 is not required for high affinity binding of purified calf uterine estrogen receptor to estrogen response element DNA  in vitro.	bind
26169	2	8047	6	13	NULL	NULL	NULL	Hsp70	GP		is not required for					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_219	11452016	4       Klinge,C.M., Brolly,C.L., Bambara,R.A. and Hilf,R. (1997) Hsp70 is not required for high affinity binding of purified calf uterine estrogen receptor to estrogen response element DNA  in vitro.	bind
31585	1	8047	7	10	NULL	0	NULL	uterine estrogen receptor	NULL	purified;;calf	bind	NULL	high affinity			DNA	NULL			estrogen response element	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_219	11452016	4       Klinge,C.M., Brolly,C.L., Bambara,R.A. and Hilf,R. (1997) Hsp70 is not required for high affinity binding of purified calf uterine estrogen receptor to estrogen response element DNA  in vitro.	bind
31586	2	8047	7	10	NULL	0	NULL	Hsp70			is not required for					statement 1					NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_219	11452016	4       Klinge,C.M., Brolly,C.L., Bambara,R.A. and Hilf,R. (1997) Hsp70 is not required for high affinity binding of purified calf uterine estrogen receptor to estrogen response element DNA  in vitro.	bind
26170	1	8048	6	13	NULL	NULL	NULL	GCN4-bZIP	GP		bind					DNA	NucleicAcid			ATF CREB site 	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3311_s_240	11504868	4       Konig,P. and Richmond,T.J. (1993) The X-ray structure of the GCN4-bZIP bound to ATF CREB site DNA shows the complex depends on DNA flexibility.	bind
26171	2	8048	6	13	NULL	NULL	NULL	statement 1	Process		depends on					DNA	NucleicAcid	flexibility of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3311_s_240	11504868	4       Konig,P. and Richmond,T.J. (1993) The X-ray structure of the GCN4-bZIP bound to ATF CREB site DNA shows the complex depends on DNA flexibility.	bind
31587	1	8048	7	NULL	NULL	0	NULL	GCN4-bZIP	NULL		bind	NULL				DNA	NULL			ATF CREB site	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3311_s_240	11504868	4       Konig,P. and Richmond,T.J. (1993) The X-ray structure of the GCN4-bZIP bound to ATF CREB site DNA shows the complex depends on DNA flexibility.	bind
31588	2	8048	7	NULL	NULL	0	NULL	statement 1	NULL		depends on	NULL				DNA 	NULL	flexibility of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3311_s_240	11504868	4       Konig,P. and Richmond,T.J. (1993) The X-ray structure of the GCN4-bZIP bound to ATF CREB site DNA shows the complex depends on DNA flexibility.	bind
26172	1	8049	6	13	NULL	NULL	NULL	NF-kappaB	GP	nuclear	bind		directly			DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jantimicrobchemoth_55_2_135_s_49	15650002	4   Electrophoretic mobility shift assays revealed that the drugs inhibit the TNF-alpha-induced DNA binding of nuclear NF-kappaB, but not the binding of NF-kappaB to DNA directly.	bind
26173	2	8049	6	13	NULL	NULL	NULL	TNF-alpha	GP		induces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jantimicrobchemoth_55_2_135_s_49	15650002	4   Electrophoretic mobility shift assays revealed that the drugs inhibit the TNF-alpha-induced DNA binding of nuclear NF-kappaB, but not the binding of NF-kappaB to DNA directly.	bind
31589	1	8049	7	NULL	NULL	0	NULL	NF-kappaB	NULL	nuclear	bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw70_jantimicrobchemoth_55_2_135_s_49	15650002	4   Electrophoretic mobility shift assays revealed that the drugs inhibit the TNF-alpha-induced DNA binding of nuclear NF-kappaB, but not the binding of NF-kappaB to DNA directly.	bind
31590	2	8049	7	NULL	NULL	0	NULL	TNF-alpha	NULL		induce	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jantimicrobchemoth_55_2_135_s_49	15650002	4   Electrophoretic mobility shift assays revealed that the drugs inhibit the TNF-alpha-induced DNA binding of nuclear NF-kappaB, but not the binding of NF-kappaB to DNA directly.	bind
26174	1	8050	6	13	NULL	NULL	NULL	p67 phox	GP		bind		poorly			Rac143Rho	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_30_18834_s_230	9228059	4   It is not clear from the Rac structure whether the poor binding of p67 phox by the Rac143Rho chimera reflects an additional binding surface for p67 phox within the 143-175 range.	bind
46539	2	8050	6	13	NULL	NULL	NULL	Rac143Rho	GP		is a type of					chimera	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_30_18834_s_230	9228059	4   It is not clear from the Rac structure whether the poor binding of p67 phox by the Rac143Rho chimera reflects an additional binding surface for p67 phox within the 143-175 range.	bind
31596	1	8050	7	10	NULL	0	NULL	Rac143Rho	NULL		bind	NULL	poorly			p67 phox	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_30_18834_s_230	9228059	4   It is not clear from the Rac structure whether the poor binding of p67 phox by the Rac143Rho chimera reflects an additional binding surface for p67 phox within the 143-175 range.	bind
46540	2	8050	7	10	NULL	0	NULL	Rac143Rho	NULL		is a type of	NULL				chimera	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_30_18834_s_230	9228059	4   It is not clear from the Rac structure whether the poor binding of p67 phox by the Rac143Rho chimera reflects an additional binding surface for p67 phox within the 143-175 range.	bind
26175	1	8051	6	13	NULL	NULL	NULL	apoE	GP		bind					Abeta-peptide	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_amjpathol_155_3_869_s_13	10487844	4  Although apoE binds Abeta-peptide and promotes beta-amyloid fibrillogenesis 5 in vitro, it is unclear whether the APOE4 genotype is associated with accelerated cognitive deterioration.	bind
26176	2	8051	6	13	NULL	NULL	NULL	statement 1	Process		promotes					beta-amyloid fibrillogenesis	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_amjpathol_155_3_869_s_13	10487844	4  Although apoE binds Abeta-peptide and promotes beta-amyloid fibrillogenesis 5 in vitro, it is unclear whether the APOE4 genotype is associated with accelerated cognitive deterioration.	bind
31599	1	8051	7	NULL	NULL	0	NULL	 apoE 	NULL		binds	NULL				Abeta-peptide	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_amjpathol_155_3_869_s_13	10487844	4  Although apoE binds Abeta-peptide and promotes beta-amyloid fibrillogenesis 5 in vitro, it is unclear whether the APOE4 genotype is associated with accelerated cognitive deterioration.	bind
31600	2	8051	7	NULL	NULL	0	NULL	statement 1	NULL		promotes	NULL				beta-amyloid fibrillogenesis	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_amjpathol_155_3_869_s_13	10487844	4  Although apoE binds Abeta-peptide and promotes beta-amyloid fibrillogenesis 5 in vitro, it is unclear whether the APOE4 genotype is associated with accelerated cognitive deterioration.	bind
26177	1	8052	6	13	NULL	NULL	NULL	MCP-1	GP		does not bind					CCR2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_6_1951_s_226	10854218	4  Another intriguing possibility is the binding of MCP-1 to receptors other than CCR2.	bind
55805	2	8052	6	13	NULL	NULL	NULL	CCR2	GP		is a type of					receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_6_1951_s_226	10854218	4  Another intriguing possibility is the binding of MCP-1 to receptors other than CCR2.	bind
31601	1	8052	7	NULL	NULL	0	NULL	MCP-1	NULL		does not bind	NULL				CCR2	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_6_1951_s_226	10854218	4  Another intriguing possibility is the binding of MCP-1 to receptors other than CCR2.	bind
31602	2	8052	7	NULL	NULL	0	NULL	CCR2	NULL		is a type of	NULL				receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_6_1951_s_226	10854218	4  Another intriguing possibility is the binding of MCP-1 to receptors other than CCR2.	bind
26178	1	8053	6	13	NULL	NULL	NULL	VSMC	Cell		is					vascular smooth muscle cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_7_648_s_6	11304484	4  Both macrophages and vascular smooth muscle cells (VSMCs) bind oxidized LDL via specific scavenger receptors, 5 6  forming foam cells.	bind
26179	2	8053	6	13	NULL	NULL	NULL	macrophages	Cell		bind					LDL	GP	oxidized			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_7_648_s_6	11304484	4  Both macrophages and vascular smooth muscle cells (VSMCs) bind oxidized LDL via specific scavenger receptors, 5 6  forming foam cells.	bind
26180	3	8053	6	13	NULL	NULL	NULL	VSMC	Cell		bind					LDL	GP	oxidized			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_7_648_s_6	11304484	4  Both macrophages and vascular smooth muscle cells (VSMCs) bind oxidized LDL via specific scavenger receptors, 5 6  forming foam cells.	bind
26181	4	8053	6	13	NULL	NULL	NULL	statement 2	Process		occurs via					scavenger receptors	GP	specific			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_7_648_s_6	11304484	4  Both macrophages and vascular smooth muscle cells (VSMCs) bind oxidized LDL via specific scavenger receptors, 5 6  forming foam cells.	bind
26182	5	8053	6	13	NULL	NULL	NULL	statement 3	Process		occurs via					scavenger receptors	GP	specific			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_7_648_s_6	11304484	4  Both macrophages and vascular smooth muscle cells (VSMCs) bind oxidized LDL via specific scavenger receptors, 5 6  forming foam cells.	bind
31603	1	8053	7	10	NULL	0	NULL	macrophages	NULL		bind	NULL				LDL	NULL	oxidized			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_7_648_s_6	11304484	4  Both macrophages and vascular smooth muscle cells (VSMCs) bind oxidized LDL via specific scavenger receptors, 5 6  forming foam cells.	bind
31604	2	8053	7	10	NULL	0	NULL	VSMCs	NULL		bind	NULL				LDL	NULL	oxidized			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_7_648_s_6	11304484	4  Both macrophages and vascular smooth muscle cells (VSMCs) bind oxidized LDL via specific scavenger receptors, 5 6  forming foam cells.	bind
31605	3	8053	7	10	NULL	0	NULL	statement 1			via					scaveger receptor		specific			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_7_648_s_6	11304484	4  Both macrophages and vascular smooth muscle cells (VSMCs) bind oxidized LDL via specific scavenger receptors, 5 6  forming foam cells.	bind
31606	4	8053	7	10	NULL	0	NULL	statement 2			via					scaveger receptor		specific			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_7_648_s_6	11304484	4  Both macrophages and vascular smooth muscle cells (VSMCs) bind oxidized LDL via specific scavenger receptors, 5 6  forming foam cells.	bind
31607	5	8053	7	NULL	NULL	0	NULL	statement 3	NULL		forms	NULL				foam cells	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_88_7_648_s_6	11304484	4  Both macrophages and vascular smooth muscle cells (VSMCs) bind oxidized LDL via specific scavenger receptors, 5 6  forming foam cells.	bind
31608	6	8053	7	NULL	NULL	0	NULL	statement 4	NULL		forms	NULL				foam cells	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_88_7_648_s_6	11304484	4  Both macrophages and vascular smooth muscle cells (VSMCs) bind oxidized LDL via specific scavenger receptors, 5 6  forming foam cells.	bind
31609	7	8053	7	NULL	NULL	0	NULL	VSMCs	NULL		is	NULL				vascular smooth muscle cells	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_88_7_648_s_6	11304484	4  Both macrophages and vascular smooth muscle cells (VSMCs) bind oxidized LDL via specific scavenger receptors, 5 6  forming foam cells.	bind
26183	1	8054	6	13	NULL	NULL	NULL	HIT antibodies	GP		bind					PF4 complexes	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_10_1479_s_16	11245656	4  HIT antibodies bind to heparin platelet factor 4 (PF4) complexes, 5  thereby activating platelets, 6 7 8  generating platelet microparticles, 9  and altering endothelial cells, 10  11 12  leading to enhanced thrombin generation and paradoxical development of new thrombi.	bind
26184	2	8054	6	13	NULL	NULL	NULL	PF4	GP		is					heparin platelet factor 4	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_10_1479_s_16	11245656	4  HIT antibodies bind to heparin platelet factor 4 (PF4) complexes, 5  thereby activating platelets, 6 7 8  generating platelet microparticles, 9  and altering endothelial cells, 10  11 12  leading to enhanced thrombin generation and paradoxical development of new thrombi.	bind
26185	3	8054	6	13	NULL	NULL	NULL	statement 1	Process		activates					platelets	Cell				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_10_1479_s_16	11245656	4  HIT antibodies bind to heparin platelet factor 4 (PF4) complexes, 5  thereby activating platelets, 6 7 8  generating platelet microparticles, 9  and altering endothelial cells, 10  11 12  leading to enhanced thrombin generation and paradoxical development of new thrombi.	bind
26186	4	8054	6	13	NULL	NULL	NULL	statement 3	Process		generates					platelet microparticles	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_10_1479_s_16	11245656	4  HIT antibodies bind to heparin platelet factor 4 (PF4) complexes, 5  thereby activating platelets, 6 7 8  generating platelet microparticles, 9  and altering endothelial cells, 10  11 12  leading to enhanced thrombin generation and paradoxical development of new thrombi.	bind
26187	5	8054	6	13	NULL	NULL	NULL	statement 4	Process		leads to					thrombin	GP	generation of;; enhanced			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_10_1479_s_16	11245656	4  HIT antibodies bind to heparin platelet factor 4 (PF4) complexes, 5  thereby activating platelets, 6 7 8  generating platelet microparticles, 9  and altering endothelial cells, 10  11 12  leading to enhanced thrombin generation and paradoxical development of new thrombi.	bind
26188	6	8054	6	13	NULL	NULL	NULL	statement 4	Process		leads to					new thrombin	GP	paradoxical development of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_10_1479_s_16	11245656	4  HIT antibodies bind to heparin platelet factor 4 (PF4) complexes, 5  thereby activating platelets, 6 7 8  generating platelet microparticles, 9  and altering endothelial cells, 10  11 12  leading to enhanced thrombin generation and paradoxical development of new thrombi.	bind
26189	7	8054	6	13	NULL	NULL	NULL	statement 1	Process		alters					endothelial cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_10_1479_s_16	11245656	4  HIT antibodies bind to heparin platelet factor 4 (PF4) complexes, 5  thereby activating platelets, 6 7 8  generating platelet microparticles, 9  and altering endothelial cells, 10  11 12  leading to enhanced thrombin generation and paradoxical development of new thrombi.	bind
31622	1	8054	7	NULL	NULL	0	NULL	HIT antibody	NULL		bind	NULL				heparin PF4 complex	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_10_1479_s_16	11245656	4  HIT antibodies bind to heparin platelet factor 4 (PF4) complexes, 5  thereby activating platelets, 6 7 8  generating platelet microparticles, 9  and altering endothelial cells, 10  11 12  leading to enhanced thrombin generation and paradoxical development of new thrombi.	bind
31623	2	8054	7	NULL	NULL	0	NULL	statement 1	NULL		activates	NULL				platelets	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_10_1479_s_16	11245656	4  HIT antibodies bind to heparin platelet factor 4 (PF4) complexes, 5  thereby activating platelets, 6 7 8  generating platelet microparticles, 9  and altering endothelial cells, 10  11 12  leading to enhanced thrombin generation and paradoxical development of new thrombi.	bind
31624	3	8054	7	NULL	NULL	0	NULL	statement 2	NULL		generate	NULL				platelet microparticles	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_10_1479_s_16	11245656	4  HIT antibodies bind to heparin platelet factor 4 (PF4) complexes, 5  thereby activating platelets, 6 7 8  generating platelet microparticles, 9  and altering endothelial cells, 10  11 12  leading to enhanced thrombin generation and paradoxical development of new thrombi.	bind
31625	4	8054	7	NULL	NULL	0	NULL	statement 3	NULL		alters	NULL				endothelial cells	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_10_1479_s_16	11245656	4  HIT antibodies bind to heparin platelet factor 4 (PF4) complexes, 5  thereby activating platelets, 6 7 8  generating platelet microparticles, 9  and altering endothelial cells, 10  11 12  leading to enhanced thrombin generation and paradoxical development of new thrombi.	bind
31626	5	8054	7	10	NULL	0	NULL	statement 4	NULL		leads to	NULL				thrombin	NULL	enhanced;;generation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_10_1479_s_16	11245656	4  HIT antibodies bind to heparin platelet factor 4 (PF4) complexes, 5  thereby activating platelets, 6 7 8  generating platelet microparticles, 9  and altering endothelial cells, 10  11 12  leading to enhanced thrombin generation and paradoxical development of new thrombi.	bind
31627	6	8054	7	NULL	NULL	0	NULL	statement 4	NULL		leads to	NULL				new thrombin	NULL	development of			NULL		0	NULL	NULL	NULL	gw60_circulation_103_10_1479_s_16	11245656	4  HIT antibodies bind to heparin platelet factor 4 (PF4) complexes, 5  thereby activating platelets, 6 7 8  generating platelet microparticles, 9  and altering endothelial cells, 10  11 12  leading to enhanced thrombin generation and paradoxical development of new thrombi.	bind
31628	7	8054	7	NULL	NULL	0	NULL	PF4	NULL		is	NULL				platelet factor 4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_10_1479_s_16	11245656	4  HIT antibodies bind to heparin platelet factor 4 (PF4) complexes, 5  thereby activating platelets, 6 7 8  generating platelet microparticles, 9  and altering endothelial cells, 10  11 12  leading to enhanced thrombin generation and paradoxical development of new thrombi.	bind
26190	1	8055	6	13	NULL	NULL	NULL	T3	Chemical		bind					T3 receptors 	GP	specific;; nuclear			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_3_260_s_8	11179190	4  In most tissues, the mechanism of TH biological action occurs by the entry of T3 into the cell by facilitated transport and the binding of T3 to specific nuclear T3 receptors (TRs), which regulate transcription of target genes.	bind
26191	2	8055	6	13	NULL	NULL	NULL	T3	Chemical		enters into					cell	Cell				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_3_260_s_8	11179190	4  In most tissues, the mechanism of TH biological action occurs by the entry of T3 into the cell by facilitated transport and the binding of T3 to specific nuclear T3 receptors (TRs), which regulate transcription of target genes.	bind
26192	3	8055	6	13	NULL	NULL	NULL	statement 2	Process		leads to					TH	Chemical	biological action of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_3_260_s_8	11179190	4  In most tissues, the mechanism of TH biological action occurs by the entry of T3 into the cell by facilitated transport and the binding of T3 to specific nuclear T3 receptors (TRs), which regulate transcription of target genes.	bind
55815	4	8055	6	13	NULL	NULL	NULL	statement 2	Process		via					facilitated transport	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_3_260_s_8	11179190	4  In most tissues, the mechanism of TH biological action occurs by the entry of T3 into the cell by facilitated transport and the binding of T3 to specific nuclear T3 receptors (TRs), which regulate transcription of target genes.	bind
55816	5	8055	6	13	NULL	NULL	NULL	TRs	GP		is					T3 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_3_260_s_8	11179190	4  In most tissues, the mechanism of TH biological action occurs by the entry of T3 into the cell by facilitated transport and the binding of T3 to specific nuclear T3 receptors (TRs), which regulate transcription of target genes.	bind
55817	6	8055	6	13	NULL	NULL	NULL	statement 1	Process		regulates					target genes	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_3_260_s_8	11179190	4  In most tissues, the mechanism of TH biological action occurs by the entry of T3 into the cell by facilitated transport and the binding of T3 to specific nuclear T3 receptors (TRs), which regulate transcription of target genes.	bind
31646	1	8055	7	NULL	NULL	0	NULL	T3	NULL		enters into the	NULL				Cell	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_3_260_s_8	11179190	4  In most tissues, the mechanism of TH biological action occurs by the entry of T3 into the cell by facilitated transport and the binding of T3 to specific nuclear T3 receptors (TRs), which regulate transcription of target genes.	bind
31647	2	8055	7	10	NULL	0	NULL	statement 1			via					facilitated transport					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_3_260_s_8	11179190	4  In most tissues, the mechanism of TH biological action occurs by the entry of T3 into the cell by facilitated transport and the binding of T3 to specific nuclear T3 receptors (TRs), which regulate transcription of target genes.	bind
31648	3	8055	7	10	NULL	0	NULL	T3	NULL		bind	NULL				T3 receptors	NULL	specific;;nuclear			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_3_260_s_8	11179190	4  In most tissues, the mechanism of TH biological action occurs by the entry of T3 into the cell by facilitated transport and the binding of T3 to specific nuclear T3 receptors (TRs), which regulate transcription of target genes.	bind
31649	4	8055	7	NULL	NULL	0	NULL	statement 3	NULL		regulate	NULL				target genes	NULL	transcription of			NULL		0	NULL	NULL	NULL	gw60_circulationres_88_3_260_s_8	11179190	4  In most tissues, the mechanism of TH biological action occurs by the entry of T3 into the cell by facilitated transport and the binding of T3 to specific nuclear T3 receptors (TRs), which regulate transcription of target genes.	bind
31650	5	8055	7	NULL	NULL	0	NULL	TRs	NULL		is	NULL				T3 receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_88_3_260_s_8	11179190	4  In most tissues, the mechanism of TH biological action occurs by the entry of T3 into the cell by facilitated transport and the binding of T3 to specific nuclear T3 receptors (TRs), which regulate transcription of target genes.	bind
55818	6	8055	7	10	NULL	0	NULL	statement 2			leads to					TH		action of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_3_260_s_8	11179190	4  In most tissues, the mechanism of TH biological action occurs by the entry of T3 into the cell by facilitated transport and the binding of T3 to specific nuclear T3 receptors (TRs), which regulate transcription of target genes.	bind
26286	1	8056	6	13	NULL	NULL	NULL	MHC	GP		repressed in					NB	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_1_291_s_236	12107114	4  In this study, we have demonstrated that the repression of MHC in NB is also caused by deficient CIITA expression and that neuroendocrine cell-specific bHLH factors competitively bind to the CIITA promoter and repress the promoter IV activity in both NB and SCLC.	bind
26287	2	8056	6	13	NULL	NULL	NULL	CIITA	GP	expression of	is deficient in					NB	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_1_291_s_236	12107114	4  In this study, we have demonstrated that the repression of MHC in NB is also caused by deficient CIITA expression and that neuroendocrine cell-specific bHLH factors competitively bind to the CIITA promoter and repress the promoter IV activity in both NB and SCLC.	bind
26288	3	8056	6	13	NULL	NULL	NULL	statement 8	GP		bind		competitively			CIITA	GP			promoter	NULL	NB	NULL	NULL	NULL	NULL	gw60_amjpathol_161_1_291_s_236	12107114	4  In this study, we have demonstrated that the repression of MHC in NB is also caused by deficient CIITA expression and that neuroendocrine cell-specific bHLH factors competitively bind to the CIITA promoter and repress the promoter IV activity in both NB and SCLC.	bind
26289	4	8056	6	13	NULL	NULL	NULL	statement 3	Process		repress					CIITA	GP	activity of		promoter IV	NULL	NB	NULL	NULL	NULL	NULL	gw60_amjpathol_161_1_291_s_236	12107114	4  In this study, we have demonstrated that the repression of MHC in NB is also caused by deficient CIITA expression and that neuroendocrine cell-specific bHLH factors competitively bind to the CIITA promoter and repress the promoter IV activity in both NB and SCLC.	bind
26290	5	8056	6	13	NULL	NULL	NULL	statement 8	GP		bind		competitively			CIITA	GP			promoter	NULL	SCLC	NULL	NULL	NULL	NULL	gw60_amjpathol_161_1_291_s_236	12107114	4  In this study, we have demonstrated that the repression of MHC in NB is also caused by deficient CIITA expression and that neuroendocrine cell-specific bHLH factors competitively bind to the CIITA promoter and repress the promoter IV activity in both NB and SCLC.	bind
26291	6	8056	6	13	NULL	NULL	NULL	statement 5	Process		repress					CIITA	GP	activity of		promoter IV	NULL	SCLC	NULL	NULL	NULL	NULL	gw60_amjpathol_161_1_291_s_236	12107114	4  In this study, we have demonstrated that the repression of MHC in NB is also caused by deficient CIITA expression and that neuroendocrine cell-specific bHLH factors competitively bind to the CIITA promoter and repress the promoter IV activity in both NB and SCLC.	bind
55819	7	8056	6	13	NULL	NULL	NULL	statement 2	Process		causes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_1_291_s_236	12107114	4  In this study, we have demonstrated that the repression of MHC in NB is also caused by deficient CIITA expression and that neuroendocrine cell-specific bHLH factors competitively bind to the CIITA promoter and repress the promoter IV activity in both NB and SCLC.	bind
55820	8	8056	6	13	NULL	NULL	NULL	bHLH factors	GP		specific to					neuroendocrine cell	Cell				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_1_291_s_236	12107114	4  In this study, we have demonstrated that the repression of MHC in NB is also caused by deficient CIITA expression and that neuroendocrine cell-specific bHLH factors competitively bind to the CIITA promoter and repress the promoter IV activity in both NB and SCLC.	bind
31651	1	8056	7	10	NULL	0	NULL	MHC			repressed in					NB					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_1_291_s_236	12107114	4  In this study, we have demonstrated that the repression of MHC in NB is also caused by deficient CIITA expression and that neuroendocrine cell-specific bHLH factors competitively bind to the CIITA promoter and repress the promoter IV activity in both NB and SCLC.	bind
31652	2	8056	7	10	NULL	0	NULL	statement 8			bind		competitively			CIITA				promoter	NULL	NB	NULL	NULL	NULL	NULL	gw60_amjpathol_161_1_291_s_236	12107114	4  In this study, we have demonstrated that the repression of MHC in NB is also caused by deficient CIITA expression and that neuroendocrine cell-specific bHLH factors competitively bind to the CIITA promoter and repress the promoter IV activity in both NB and SCLC.	bind
31653	3	8056	7	10	NULL	0	NULL	statement 8			bind		competitively			CIITA				promoter	NULL	SCLC	NULL	NULL	NULL	NULL	gw60_amjpathol_161_1_291_s_236	12107114	4  In this study, we have demonstrated that the repression of MHC in NB is also caused by deficient CIITA expression and that neuroendocrine cell-specific bHLH factors competitively bind to the CIITA promoter and repress the promoter IV activity in both NB and SCLC.	bind
31655	4	8056	7	NULL	NULL	0	NULL	statement 2	NULL		repress	NULL					NULL	activity of		promoter IV	NULL	NB	0	NULL	NULL	NULL	gw60_amjpathol_161_1_291_s_236	12107114	4  In this study, we have demonstrated that the repression of MHC in NB is also caused by deficient CIITA expression and that neuroendocrine cell-specific bHLH factors competitively bind to the CIITA promoter and repress the promoter IV activity in both NB and SCLC.	bind
31657	5	8056	7	NULL	NULL	0	NULL	statement 3	NULL		repress	NULL					NULL	activity of		promoter IV	NULL	SCLC	0	NULL	NULL	NULL	gw60_amjpathol_161_1_291_s_236	12107114	4  In this study, we have demonstrated that the repression of MHC in NB is also caused by deficient CIITA expression and that neuroendocrine cell-specific bHLH factors competitively bind to the CIITA promoter and repress the promoter IV activity in both NB and SCLC.	bind
55821	6	8056	7	10	NULL	0	NULL	CIITA		expression of	is deficient in					NB					NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_1_291_s_236	12107114	4  In this study, we have demonstrated that the repression of MHC in NB is also caused by deficient CIITA expression and that neuroendocrine cell-specific bHLH factors competitively bind to the CIITA promoter and repress the promoter IV activity in both NB and SCLC.	bind
55822	7	8056	7	10	NULL	0	NULL	statement 6			causes					statement 1					NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_1_291_s_236	12107114	4  In this study, we have demonstrated that the repression of MHC in NB is also caused by deficient CIITA expression and that neuroendocrine cell-specific bHLH factors competitively bind to the CIITA promoter and repress the promoter IV activity in both NB and SCLC.	bind
55823	8	8056	7	10	NULL	0	NULL	bHLH factors			specific to					neuroendocrine cell					NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_1_291_s_236	12107114	4  In this study, we have demonstrated that the repression of MHC in NB is also caused by deficient CIITA expression and that neuroendocrine cell-specific bHLH factors competitively bind to the CIITA promoter and repress the promoter IV activity in both NB and SCLC.	bind
26193	1	8057	6	13	NULL	NULL	NULL	fibrinogen	GP		bind					platelet GP IIb/IIa receptor	GP	activated			NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_2_149_s_21	10889124	4  Orbofiban is an oral ethyl-ester pro-drug that specifically blocks the binding of fibrinogen to the platelet GP IIb/IIa receptor (with a higher affinity for the activated versus unactivated receptor), thereby interfering with the platelet aggregation induced by various agonists.	bind
26194	2	8057	6	13	NULL	NULL	NULL	Orbofiban	Chemical		blocks 		specifically			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_2_149_s_21	10889124	4  Orbofiban is an oral ethyl-ester pro-drug that specifically blocks the binding of fibrinogen to the platelet GP IIb/IIa receptor (with a higher affinity for the activated versus unactivated receptor), thereby interfering with the platelet aggregation induced by various agonists.	bind
26195	3	8057	6	13	NULL	NULL	NULL	Orbofiban	Chemical		is a type of					oral ethyl-ester pro-drug	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_2_149_s_21	10889124	4  Orbofiban is an oral ethyl-ester pro-drug that specifically blocks the binding of fibrinogen to the platelet GP IIb/IIa receptor (with a higher affinity for the activated versus unactivated receptor), thereby interfering with the platelet aggregation induced by various agonists.	bind
26196	4	8057	6	13	NULL	NULL	NULL	fibrinogen	GP		bind					platelet glycoprotein IIb/IIa complex	GP	unactivated			NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_2_149_s_21	10889124	4  Orbofiban is an oral ethyl-ester pro-drug that specifically blocks the binding of fibrinogen to the platelet GP IIb/IIa receptor (with a higher affinity for the activated versus unactivated receptor), thereby interfering with the platelet aggregation induced by various agonists.	bind
26197	5	8057	6	13	NULL	NULL	NULL	statement 1	Process	affinity of	is higher than					statement 4	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_2_149_s_21	10889124	4  Orbofiban is an oral ethyl-ester pro-drug that specifically blocks the binding of fibrinogen to the platelet GP IIb/IIa receptor (with a higher affinity for the activated versus unactivated receptor), thereby interfering with the platelet aggregation induced by various agonists.	bind
26198	6	8057	6	13	NULL	NULL	NULL	statement 2	Process		interferes with					platelet aggregation	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_2_149_s_21	10889124	4  Orbofiban is an oral ethyl-ester pro-drug that specifically blocks the binding of fibrinogen to the platelet GP IIb/IIa receptor (with a higher affinity for the activated versus unactivated receptor), thereby interfering with the platelet aggregation induced by various agonists.	bind
31661	1	8057	7	NULL	NULL	0	NULL	fibrinogen	NULL		bind	NULL	high affinity			GP IIb/IIa receptor	NULL	activated			NULL		0	NULL	NULL	NULL	gw60_circulation_102_2_149_s_21	10889124	4  Orbofiban is an oral ethyl-ester pro-drug that specifically blocks the binding of fibrinogen to the platelet GP IIb/IIa receptor (with a higher affinity for the activated versus unactivated receptor), thereby interfering with the platelet aggregation induced by various agonists.	bind
31664	2	8057	7	NULL	NULL	0	NULL	fibrinogen	NULL		bind	NULL				platelet GP IIb/IIa receptor	NULL	unactivated			NULL		0	NULL	NULL	NULL	gw60_circulation_102_2_149_s_21	10889124	4  Orbofiban is an oral ethyl-ester pro-drug that specifically blocks the binding of fibrinogen to the platelet GP IIb/IIa receptor (with a higher affinity for the activated versus unactivated receptor), thereby interfering with the platelet aggregation induced by various agonists.	bind
31665	3	8057	7	10	NULL	0	NULL	statement 1	NULL		higher affinity than	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_2_149_s_21	10889124	4  Orbofiban is an oral ethyl-ester pro-drug that specifically blocks the binding of fibrinogen to the platelet GP IIb/IIa receptor (with a higher affinity for the activated versus unactivated receptor), thereby interfering with the platelet aggregation induced by various agonists.	bind
31667	4	8057	7	NULL	NULL	0	NULL	Orbofiban	NULL		blocks	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_102_2_149_s_21	10889124	4  Orbofiban is an oral ethyl-ester pro-drug that specifically blocks the binding of fibrinogen to the platelet GP IIb/IIa receptor (with a higher affinity for the activated versus unactivated receptor), thereby interfering with the platelet aggregation induced by various agonists.	bind
31668	5	8057	7	NULL	NULL	0	NULL	Orbofiban	NULL		blocks	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_102_2_149_s_21	10889124	4  Orbofiban is an oral ethyl-ester pro-drug that specifically blocks the binding of fibrinogen to the platelet GP IIb/IIa receptor (with a higher affinity for the activated versus unactivated receptor), thereby interfering with the platelet aggregation induced by various agonists.	bind
31671	6	8057	7	NULL	NULL	0	NULL	Orbofiban	NULL		is a type of	NULL				oral ethyl-ester pro-drug	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_102_2_149_s_21	10889124	4  Orbofiban is an oral ethyl-ester pro-drug that specifically blocks the binding of fibrinogen to the platelet GP IIb/IIa receptor (with a higher affinity for the activated versus unactivated receptor), thereby interfering with the platelet aggregation induced by various agonists.	bind
31673	7	8057	7	NULL	NULL	0	NULL	agonists	NULL		induce	NULL				platelet aggregation	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_102_2_149_s_21	10889124	4  Orbofiban is an oral ethyl-ester pro-drug that specifically blocks the binding of fibrinogen to the platelet GP IIb/IIa receptor (with a higher affinity for the activated versus unactivated receptor), thereby interfering with the platelet aggregation induced by various agonists.	bind
31675	8	8057	7	NULL	NULL	0	NULL	Orbofiban	NULL		interferes with	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_102_2_149_s_21	10889124	4  Orbofiban is an oral ethyl-ester pro-drug that specifically blocks the binding of fibrinogen to the platelet GP IIb/IIa receptor (with a higher affinity for the activated versus unactivated receptor), thereby interfering with the platelet aggregation induced by various agonists.	bind
26199	1	8058	6	13	NULL	NULL	NULL	Cdc24	GP		bind		directly			Ste5	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_13_13084_s_214	15657049	4  These data substantiate the evidence that Cdc24 binds directly to Ste5 and argue that Cdc24-Ste5 complexes are distinct from Cdc24-Far1 complexes.	bind
46541	2	8058	6	13	NULL	NULL	NULL	Cdc24-Ste5 complex	GP		is distinct from					Cdc24-Far1 complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_13_13084_s_214	15657049	4  These data substantiate the evidence that Cdc24 binds directly to Ste5 and argue that Cdc24-Ste5 complexes are distinct from Cdc24-Far1 complexes.	bind
31676	1	8058	7	NULL	NULL	0	NULL	Cdc24	NULL		binds	NULL	directly			 Ste5	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_13_13084_s_214	15657049	4  These data substantiate the evidence that Cdc24 binds directly to Ste5 and argue that Cdc24-Ste5 complexes are distinct from Cdc24-Far1 complexes.	bind
31677	2	8058	7	NULL	NULL	0	NULL	Cdc24-Ste5 complex	NULL		is distinct from	NULL				Cdc24-Far1 complex	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_13_13084_s_214	15657049	4  These data substantiate the evidence that Cdc24 binds directly to Ste5 and argue that Cdc24-Ste5 complexes are distinct from Cdc24-Far1 complexes.	bind
26200	1	8059	6	13	NULL	NULL	NULL	vWF	GP		bind					GP Ib	GP	platelet			NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_6_1399_s_19	7664419	4  vWf must bind to both platelet GP Ib and GP IIb/IIa to support full platelet aggregation at these elevated levels of shear stress.	bind
26201	2	8059	6	13	NULL	NULL	NULL	vWF	GP		bind					GP IIb/IIa	GP	platelet			NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_6_1399_s_19	7664419	4  vWf must bind to both platelet GP Ib and GP IIb/IIa to support full platelet aggregation at these elevated levels of shear stress.	bind
26202	3	8059	6	13	NULL	NULL	NULL	statement 1	Process		occurs along with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_6_1399_s_19	7664419	4  vWf must bind to both platelet GP Ib and GP IIb/IIa to support full platelet aggregation at these elevated levels of shear stress.	bind
26203	4	8059	6	13	NULL	NULL	NULL	statement 3	Process		support					platelet	Cell	aggregation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_6_1399_s_19	7664419	4  vWf must bind to both platelet GP Ib and GP IIb/IIa to support full platelet aggregation at these elevated levels of shear stress.	bind
31678	1	8059	7	10	NULL	0	NULL	vWf			bind					GP Ib 		platelet			NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_6_1399_s_19	7664419	4  vWf must bind to both platelet GP Ib and GP IIb/IIa to support full platelet aggregation at these elevated levels of shear stress.	bind
31679	2	8059	7	10	NULL	0	NULL	vWF			bind					GP IIb/IIa		platelet			NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_6_1399_s_19	7664419	4  vWf must bind to both platelet GP Ib and GP IIb/IIa to support full platelet aggregation at these elevated levels of shear stress.	bind
31680	3	8059	7	NULL	NULL	0	NULL	statement 1	NULL		occurs along with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_6_1399_s_19	7664419	4  vWf must bind to both platelet GP Ib and GP IIb/IIa to support full platelet aggregation at these elevated levels of shear stress.	bind
31681	4	8059	7	10	NULL	0	NULL	statement 3			support					platelet		aggregation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_6_1399_s_19	7664419	4  vWf must bind to both platelet GP Ib and GP IIb/IIa to support full platelet aggregation at these elevated levels of shear stress.	bind
31682	5	8059	7	NULL	NULL	0	NULL	statement 4	NULL		occurs at	NULL				shear stress	NULL	elevated levels of			NULL		0	NULL	NULL	NULL	gw60_circulation_92_6_1399_s_19	7664419	4  vWf must bind to both platelet GP Ib and GP IIb/IIa to support full platelet aggregation at these elevated levels of shear stress.	bind
26204	1	8060	6	13	NULL	NULL	NULL	apoE2	GP		bind					LDLR	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_91_s_22	12969990	4 - 6   Additionally, individuals homozygous for apoE2, which binds to the LDLR with much less affinity than either apoE3 or apoE4, have low plasma cholesterol and are generally protected from atherosclerosis, except for the 5% to 10% of apoE2 homozygotes who develop type III hyperlipoproteinemia.	bind
26205	2	8060	6	13	NULL	NULL	NULL	apoE3	GP		bind					LDLR	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_91_s_22	12969990	4 - 6   Additionally, individuals homozygous for apoE2, which binds to the LDLR with much less affinity than either apoE3 or apoE4, have low plasma cholesterol and are generally protected from atherosclerosis, except for the 5% to 10% of apoE2 homozygotes who develop type III hyperlipoproteinemia.	bind
26206	3	8060	6	13	NULL	NULL	NULL	apoE4	GP		bind					LDLR	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_91_s_22	12969990	4 - 6   Additionally, individuals homozygous for apoE2, which binds to the LDLR with much less affinity than either apoE3 or apoE4, have low plasma cholesterol and are generally protected from atherosclerosis, except for the 5% to 10% of apoE2 homozygotes who develop type III hyperlipoproteinemia.	bind
26207	4	8060	6	13	NULL	NULL	NULL	statement 1	Process	affinity of	is less than					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_91_s_22	12969990	4 - 6   Additionally, individuals homozygous for apoE2, which binds to the LDLR with much less affinity than either apoE3 or apoE4, have low plasma cholesterol and are generally protected from atherosclerosis, except for the 5% to 10% of apoE2 homozygotes who develop type III hyperlipoproteinemia.	bind
26208	5	8060	6	13	NULL	NULL	NULL	statement 1	Process	affinity of	is less than					statement 3	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_91_s_22	12969990	4 - 6   Additionally, individuals homozygous for apoE2, which binds to the LDLR with much less affinity than either apoE3 or apoE4, have low plasma cholesterol and are generally protected from atherosclerosis, except for the 5% to 10% of apoE2 homozygotes who develop type III hyperlipoproteinemia.	bind
26209	6	8060	6	13	NULL	NULL	NULL	homozygous apoE2	Organism	human	correlates with					plasma cholesterol	Chemical	low levels of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_91_s_22	12969990	4 - 6   Additionally, individuals homozygous for apoE2, which binds to the LDLR with much less affinity than either apoE3 or apoE4, have low plasma cholesterol and are generally protected from atherosclerosis, except for the 5% to 10% of apoE2 homozygotes who develop type III hyperlipoproteinemia.	bind
26210	7	8060	6	13	NULL	NULL	NULL	homozygous apoE2	Organism	human	are protected from					atherosclerosis	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_91_s_22	12969990	4 - 6   Additionally, individuals homozygous for apoE2, which binds to the LDLR with much less affinity than either apoE3 or apoE4, have low plasma cholesterol and are generally protected from atherosclerosis, except for the 5% to 10% of apoE2 homozygotes who develop type III hyperlipoproteinemia.	bind
26211	8	8060	6	13	NULL	NULL	NULL	apoE2 homozygotes	Organism		develop					type III hyperlipoproteinemia	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_91_s_22	12969990	4 - 6   Additionally, individuals homozygous for apoE2, which binds to the LDLR with much less affinity than either apoE3 or apoE4, have low plasma cholesterol and are generally protected from atherosclerosis, except for the 5% to 10% of apoE2 homozygotes who develop type III hyperlipoproteinemia.	bind
31719	1	8060	7	NULL	NULL	0	NULL	apoE2	NULL		binds	NULL	less affinity			LDLR	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_91_s_22	12969990	4 - 6   Additionally, individuals homozygous for apoE2, which binds to the LDLR with much less affinity than either apoE3 or apoE4, have low plasma cholesterol and are generally protected from atherosclerosis, except for the 5% to 10% of apoE2 homozygotes who develop type III hyperlipoproteinemia.	bind
31720	2	8060	7	NULL	NULL	0	NULL	apoE3	NULL		binds	NULL				LDLR	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_91_s_22	12969990	4 - 6   Additionally, individuals homozygous for apoE2, which binds to the LDLR with much less affinity than either apoE3 or apoE4, have low plasma cholesterol and are generally protected from atherosclerosis, except for the 5% to 10% of apoE2 homozygotes who develop type III hyperlipoproteinemia.	bind
31721	3	8060	7	NULL	NULL	0	NULL	apoE4	NULL		binds	NULL				LDLR	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_91_s_22	12969990	4 - 6   Additionally, individuals homozygous for apoE2, which binds to the LDLR with much less affinity than either apoE3 or apoE4, have low plasma cholesterol and are generally protected from atherosclerosis, except for the 5% to 10% of apoE2 homozygotes who develop type III hyperlipoproteinemia.	bind
31722	4	8060	7	10	NULL	0	NULL	statement 2	NULL		lower affinity than	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_91_s_22	12969990	4 - 6   Additionally, individuals homozygous for apoE2, which binds to the LDLR with much less affinity than either apoE3 or apoE4, have low plasma cholesterol and are generally protected from atherosclerosis, except for the 5% to 10% of apoE2 homozygotes who develop type III hyperlipoproteinemia.	bind
31723	5	8060	7	10	NULL	0	NULL	statement 3	NULL		lower affinity than	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_91_s_22	12969990	4 - 6   Additionally, individuals homozygous for apoE2, which binds to the LDLR with much less affinity than either apoE3 or apoE4, have low plasma cholesterol and are generally protected from atherosclerosis, except for the 5% to 10% of apoE2 homozygotes who develop type III hyperlipoproteinemia.	bind
31724	6	8060	7	NULL	NULL	0	NULL	plasma cholesterol	NULL		is less in	NULL				homozygous apoE2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_91_s_22	12969990	4 - 6   Additionally, individuals homozygous for apoE2, which binds to the LDLR with much less affinity than either apoE3 or apoE4, have low plasma cholesterol and are generally protected from atherosclerosis, except for the 5% to 10% of apoE2 homozygotes who develop type III hyperlipoproteinemia.	bind
31725	7	8060	7	NULL	NULL	0	NULL	statement 6	NULL		protects from	NULL				atherosclerosis	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_1_91_s_22	12969990	4 - 6   Additionally, individuals homozygous for apoE2, which binds to the LDLR with much less affinity than either apoE3 or apoE4, have low plasma cholesterol and are generally protected from atherosclerosis, except for the 5% to 10% of apoE2 homozygotes who develop type III hyperlipoproteinemia.	bind
26292	1	8061	6	13	NULL	NULL	NULL	LDL receptor	GP		mediates					LDL particles	GP	uptake of 			NULL	in liver	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2376_s_17	9409204	4 - 6 A deletion of four amino acids from the cysteine-rich ligand binding domain of the LDL receptor7,8 preventing the LDL receptor-mediated uptake of LDL particles in the liver results in a dramatic increase of LDL cholesterol that is associated with accelerated atherosclerosis.	bind
26293	2	8061	6	13	NULL	NULL	NULL	statement 5	AminoAcid		prevents					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2376_s_17	9409204	4 - 6 A deletion of four amino acids from the cysteine-rich ligand binding domain of the LDL receptor7,8 preventing the LDL receptor-mediated uptake of LDL particles in the liver results in a dramatic increase of LDL cholesterol that is associated with accelerated atherosclerosis.	bind
26294	3	8061	6	13	NULL	NULL	NULL	statement 2	Process		results in					LDL cholesterol	Chemical	increase in			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2376_s_17	9409204	4 - 6 A deletion of four amino acids from the cysteine-rich ligand binding domain of the LDL receptor7,8 preventing the LDL receptor-mediated uptake of LDL particles in the liver results in a dramatic increase of LDL cholesterol that is associated with accelerated atherosclerosis.	bind
26295	4	8061	6	13	NULL	NULL	NULL	statement 3	Process		is associated with					atherosclerosis	MedicalFinding	accelerated			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2376_s_17	9409204	4 - 6 A deletion of four amino acids from the cysteine-rich ligand binding domain of the LDL receptor7,8 preventing the LDL receptor-mediated uptake of LDL particles in the liver results in a dramatic increase of LDL cholesterol that is associated with accelerated atherosclerosis.	bind
55824	5	8061	6	13	NULL	NULL	NULL	four amino acids	AminoAcid		deleted from					LDL receptor	GP		cysteine-rich ligand binding domain		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2376_s_17	9409204	4 - 6 A deletion of four amino acids from the cysteine-rich ligand binding domain of the LDL receptor7,8 preventing the LDL receptor-mediated uptake of LDL particles in the liver results in a dramatic increase of LDL cholesterol that is associated with accelerated atherosclerosis.	bind
31726	1	8061	7	NULL	NULL	0	NULL	LDL receptor	NULL		mediates	NULL				LDL particles	NULL	uptake of			NULL	in the liver	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2376_s_17	9409204	4 - 6 A deletion of four amino acids from the cysteine-rich ligand binding domain of the LDL receptor7,8 preventing the LDL receptor-mediated uptake of LDL particles in the liver results in a dramatic increase of LDL cholesterol that is associated with accelerated atherosclerosis.	bind
31727	2	8061	7	10	NULL	0	NULL	statement 5			prevents					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2376_s_17	9409204	4 - 6 A deletion of four amino acids from the cysteine-rich ligand binding domain of the LDL receptor7,8 preventing the LDL receptor-mediated uptake of LDL particles in the liver results in a dramatic increase of LDL cholesterol that is associated with accelerated atherosclerosis.	bind
31728	3	8061	7	NULL	NULL	0	NULL	statement 2	NULL		increase	NULL				LDL cholesterol	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2376_s_17	9409204	4 - 6 A deletion of four amino acids from the cysteine-rich ligand binding domain of the LDL receptor7,8 preventing the LDL receptor-mediated uptake of LDL particles in the liver results in a dramatic increase of LDL cholesterol that is associated with accelerated atherosclerosis.	bind
31729	4	8061	7	NULL	NULL	0	NULL	statement 3	NULL		is associated with	NULL				atherosclerosis	NULL	accelerated			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2376_s_17	9409204	4 - 6 A deletion of four amino acids from the cysteine-rich ligand binding domain of the LDL receptor7,8 preventing the LDL receptor-mediated uptake of LDL particles in the liver results in a dramatic increase of LDL cholesterol that is associated with accelerated atherosclerosis.	bind
55825	5	8061	7	10	NULL	0	NULL	four amino acids			deleted from					LDL receptor			cysteine-rich ligand binding domain		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2376_s_17	9409204	4 - 6 A deletion of four amino acids from the cysteine-rich ligand binding domain of the LDL receptor7,8 preventing the LDL receptor-mediated uptake of LDL particles in the liver results in a dramatic increase of LDL cholesterol that is associated with accelerated atherosclerosis.	bind
26212	1	8062	6	13	NULL	NULL	NULL	CrkL	GP		bind					Cbl	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_301_4_934_s_40	12589802	4 1 Integrin cross-linking induces tyrosine phosphorylation of Cbl, Pyk2,  and Shc as well as binding of CrkL with Cbl. 32D/EpoR-Wt cells were starved overnight  from Epo and then stimulated by cross-linking with anti- 4 antibody for 15 min or  for the indicated times at 37  degrees C before solubilization.	bind
26213	2	8062	6	13	NULL	NULL	NULL	integrin	GP	crosslinking of	induces					Cbl	GP	phosphorylation of	tyrosine		NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_301_4_934_s_40	12589802	4 1 Integrin cross-linking induces tyrosine phosphorylation of Cbl, Pyk2,  and Shc as well as binding of CrkL with Cbl. 32D/EpoR-Wt cells were starved overnight  from Epo and then stimulated by cross-linking with anti- 4 antibody for 15 min or  for the indicated times at 37  degrees C before solubilization.	bind
26214	3	8062	6	13	NULL	NULL	NULL	integrin	GP	crosslinking of	induces					Pyk2	GP	phosphorylation of	tyrosine		NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_301_4_934_s_40	12589802	4 1 Integrin cross-linking induces tyrosine phosphorylation of Cbl, Pyk2,  and Shc as well as binding of CrkL with Cbl. 32D/EpoR-Wt cells were starved overnight  from Epo and then stimulated by cross-linking with anti- 4 antibody for 15 min or  for the indicated times at 37  degrees C before solubilization.	bind
26215	4	8062	6	13	NULL	NULL	NULL	integrin	GP	crosslinking of	induces					Shc	GP	phosphorylation of	tyrosine		NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_301_4_934_s_40	12589802	4 1 Integrin cross-linking induces tyrosine phosphorylation of Cbl, Pyk2,  and Shc as well as binding of CrkL with Cbl. 32D/EpoR-Wt cells were starved overnight  from Epo and then stimulated by cross-linking with anti- 4 antibody for 15 min or  for the indicated times at 37  degrees C before solubilization.	bind
26216	5	8062	6	13	NULL	NULL	NULL	integrin	GP	crosslinking of	induces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_301_4_934_s_40	12589802	4 1 Integrin cross-linking induces tyrosine phosphorylation of Cbl, Pyk2,  and Shc as well as binding of CrkL with Cbl. 32D/EpoR-Wt cells were starved overnight  from Epo and then stimulated by cross-linking with anti- 4 antibody for 15 min or  for the indicated times at 37  degrees C before solubilization.	bind
31730	1	8062	7	NULL	NULL	0	NULL	Integrin	NULL	 cross-linking of	induce	NULL				Cbl	NULL	phosphorylation of	tyrosine		NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_301_4_934_s_40	12589802	4 1 Integrin cross-linking induces tyrosine phosphorylation of Cbl, Pyk2,  and Shc as well as binding of CrkL with Cbl. 32D/EpoR-Wt cells were starved overnight  from Epo and then stimulated by cross-linking with anti- 4 antibody for 15 min or  for the indicated times at 37  degrees C before solubilization.	bind
31731	2	8062	7	NULL	NULL	0	NULL	Integrin	NULL	cross-linking of	induce	NULL				Pyk2	NULL	phosphorylation of	tyrosine		NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_301_4_934_s_40	12589802	4 1 Integrin cross-linking induces tyrosine phosphorylation of Cbl, Pyk2,  and Shc as well as binding of CrkL with Cbl. 32D/EpoR-Wt cells were starved overnight  from Epo and then stimulated by cross-linking with anti- 4 antibody for 15 min or  for the indicated times at 37  degrees C before solubilization.	bind
31732	3	8062	7	NULL	NULL	0	NULL	Integrin	NULL	cross-linking of	induce	NULL				Shc	NULL	phosphorylation of	tyrosine		NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_301_4_934_s_40	12589802	4 1 Integrin cross-linking induces tyrosine phosphorylation of Cbl, Pyk2,  and Shc as well as binding of CrkL with Cbl. 32D/EpoR-Wt cells were starved overnight  from Epo and then stimulated by cross-linking with anti- 4 antibody for 15 min or  for the indicated times at 37  degrees C before solubilization.	bind
31733	4	8062	7	NULL	NULL	0	NULL	CrkL	NULL		bind	NULL				Cbl	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_301_4_934_s_40	12589802	4 1 Integrin cross-linking induces tyrosine phosphorylation of Cbl, Pyk2,  and Shc as well as binding of CrkL with Cbl. 32D/EpoR-Wt cells were starved overnight  from Epo and then stimulated by cross-linking with anti- 4 antibody for 15 min or  for the indicated times at 37  degrees C before solubilization.	bind
26217	1	8064	6	13	NULL	NULL	NULL	CGP 12177	Chemical	3H-labeled	bind					beta2-adrenoceptors	GP				NULL	CHO-beta2 cells	NULL	NULL	NULL	NULL	gw60_brjpharmacol_137_3_400_s_7	12237261	4 3H-CGP 12177 binding to beta2-adrenoceptors in intact CHO-beta2 cells yielded a log  K D value of -9.84 plus-or-minus 0.06, but indicated that the ligand dissociates very slowly from the receptor (t  for dissociation=65 min).	bind
31734	1	8064	7	10	NULL	0	NULL	CGP 12177		3H-labeled	bind					beta2-adrenoceptors					NULL	intact CHO-beta2 cells	NULL	NULL	NULL	NULL	gw60_brjpharmacol_137_3_400_s_7	12237261	4 3H-CGP 12177 binding to beta2-adrenoceptors in intact CHO-beta2 cells yielded a log  K D value of -9.84 plus-or-minus 0.06, but indicated that the ligand dissociates very slowly from the receptor (t  for dissociation=65 min).	bind
26218	1	8065	6	13	NULL	NULL	NULL	ETA receptors	GP		bind					endothelin-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_94_3_316_s_124	8759071	4 5  8 11  ETA receptors bind endothelin-1 and, to a lesser degree, endothelin-3; ETB receptors bind endothelin-1 and endothelin-3 with similar affinity.	bind
26219	2	8065	6	13	NULL	NULL	NULL	ETA receptors	GP		bind					endothelin-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_94_3_316_s_124	8759071	4 5  8 11  ETA receptors bind endothelin-1 and, to a lesser degree, endothelin-3; ETB receptors bind endothelin-1 and endothelin-3 with similar affinity.	bind
26220	3	8065	6	13	NULL	NULL	NULL	statement 1	Process	affinity of	is higher than					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_94_3_316_s_124	8759071	4 5  8 11  ETA receptors bind endothelin-1 and, to a lesser degree, endothelin-3; ETB receptors bind endothelin-1 and endothelin-3 with similar affinity.	bind
26221	4	8065	6	13	NULL	NULL	NULL	ETB receptor	GP		bind					endothelin-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_94_3_316_s_124	8759071	4 5  8 11  ETA receptors bind endothelin-1 and, to a lesser degree, endothelin-3; ETB receptors bind endothelin-1 and endothelin-3 with similar affinity.	bind
26222	5	8065	6	13	NULL	NULL	NULL	ETB receptor	GP		bind					endothelin-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_94_3_316_s_124	8759071	4 5  8 11  ETA receptors bind endothelin-1 and, to a lesser degree, endothelin-3; ETB receptors bind endothelin-1 and endothelin-3 with similar affinity.	bind
26223	6	8065	6	13	NULL	NULL	NULL	statement 4	Process	affinity of	is equal to					statement 5	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_94_3_316_s_124	8759071	4 5  8 11  ETA receptors bind endothelin-1 and, to a lesser degree, endothelin-3; ETB receptors bind endothelin-1 and endothelin-3 with similar affinity.	bind
31737	1	8065	7	NULL	NULL	0	NULL	ETA receptors	NULL		bind	NULL				endothelin-1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_94_3_316_s_124	8759071	4 5  8 11  ETA receptors bind endothelin-1 and, to a lesser degree, endothelin-3; ETB receptors bind endothelin-1 and endothelin-3 with similar affinity.	bind
31738	2	8065	7	NULL	NULL	0	NULL	ETA receptors	NULL		bind	NULL				endothelin-3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_94_3_316_s_124	8759071	4 5  8 11  ETA receptors bind endothelin-1 and, to a lesser degree, endothelin-3; ETB receptors bind endothelin-1 and endothelin-3 with similar affinity.	bind
31739	3	8065	7	NULL	NULL	0	NULL	statement 2	NULL	binding of	is less than	NULL				statement 1	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_circulation_94_3_316_s_124	8759071	4 5  8 11  ETA receptors bind endothelin-1 and, to a lesser degree, endothelin-3; ETB receptors bind endothelin-1 and endothelin-3 with similar affinity.	bind
31740	4	8065	7	NULL	NULL	0	NULL	ETB receptors 	NULL		bind	NULL				endothelin-1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_94_3_316_s_124	8759071	4 5  8 11  ETA receptors bind endothelin-1 and, to a lesser degree, endothelin-3; ETB receptors bind endothelin-1 and endothelin-3 with similar affinity.	bind
31741	5	8065	7	NULL	NULL	0	NULL	ETB receptors	NULL		bind	NULL				endothelin-3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_94_3_316_s_124	8759071	4 5  8 11  ETA receptors bind endothelin-1 and, to a lesser degree, endothelin-3; ETB receptors bind endothelin-1 and endothelin-3 with similar affinity.	bind
31742	6	8065	7	NULL	NULL	0	NULL	statement 4	NULL	affinity of	is similar to	NULL				statement 5	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw60_circulation_94_3_316_s_124	8759071	4 5  8 11  ETA receptors bind endothelin-1 and, to a lesser degree, endothelin-3; ETB receptors bind endothelin-1 and endothelin-3 with similar affinity.	bind
26224	1	8066	6	13	NULL	NULL	NULL	P1GF homodimer	GP		bind		only			Flt-1 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_93_8_1493_s_60	8608615	4 5  The PlGF homodimer binds only to the Flt-1 receptor.	bind
31743	1	8066	7	10	NULL	0	NULL	 PlGF homodimer			binds		only			Flt-1 receptor					NULL		NULL	NULL	NULL	NULL	gw60_circulation_93_8_1493_s_60	8608615	4 5  The PlGF homodimer binds only to the Flt-1 receptor.	bind
26225	1	8068	6	13	NULL	NULL	NULL	MyBP-C	GP		bind					myosin subfragment-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_9_841_s_20	10532952	4 5 6  MyBP-C binds with myosin subfragment-2 and light meromyosin 7  and also interacts with titin (or connectin).	bind
26226	2	8068	6	13	NULL	NULL	NULL	MyBP-C	GP		bind					light meromyosin 7	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_9_841_s_20	10532952	4 5 6  MyBP-C binds with myosin subfragment-2 and light meromyosin 7  and also interacts with titin (or connectin).	bind
26227	3	8068	6	13	NULL	NULL	NULL	MyBP-C	GP		interacts with					titin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_9_841_s_20	10532952	4 5 6  MyBP-C binds with myosin subfragment-2 and light meromyosin 7  and also interacts with titin (or connectin).	bind
26228	4	8068	6	13	NULL	NULL	NULL	MyBP-C	GP		interacts with					connectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_9_841_s_20	10532952	4 5 6  MyBP-C binds with myosin subfragment-2 and light meromyosin 7  and also interacts with titin (or connectin).	bind
26229	5	8068	6	13	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_9_841_s_20	10532952	4 5 6  MyBP-C binds with myosin subfragment-2 and light meromyosin 7  and also interacts with titin (or connectin).	bind
31746	1	8068	7	NULL	NULL	0	NULL	MyBP-C	NULL		binds	NULL				myosin subfragment-2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_85_9_841_s_20	10532952	4 5 6  MyBP-C binds with myosin subfragment-2 and light meromyosin 7  and also interacts with titin (or connectin).	bind
31747	2	8068	7	NULL	NULL	0	NULL	MyBP-C 	NULL		binds	NULL				light meromyosin 7	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_85_9_841_s_20	10532952	4 5 6  MyBP-C binds with myosin subfragment-2 and light meromyosin 7  and also interacts with titin (or connectin).	bind
31748	3	8068	7	NULL	NULL	0	NULL	MyBP-C	NULL		interacts with	NULL				titin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_85_9_841_s_20	10532952	4 5 6  MyBP-C binds with myosin subfragment-2 and light meromyosin 7  and also interacts with titin (or connectin).	bind
31749	4	8068	7	NULL	NULL	0	NULL	MyBP-C	NULL		interacts with	NULL				connectin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_9_841_s_20	10532952	4 5 6  MyBP-C binds with myosin subfragment-2 and light meromyosin 7  and also interacts with titin (or connectin).	bind
26230	1	8069	6	13	NULL	NULL	NULL	fibrinogen	GP		bind					ADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_156_s_35	9012651	4 5 6 7 8 9 10 11 12 13 14 15 16 17 18  Furthermore, instead of inducing inhibition, LDL particles increased the binding of fibrinogen to both ADP and proteolytic enzyme - activated platelets.	bind
26231	2	8069	6	13	NULL	NULL	NULL	fibrinogen	GP		bind					platelets	Cell	proteolytic enzyme - activated			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_156_s_35	9012651	4 5 6 7 8 9 10 11 12 13 14 15 16 17 18  Furthermore, instead of inducing inhibition, LDL particles increased the binding of fibrinogen to both ADP and proteolytic enzyme - activated platelets.	bind
26232	3	8069	6	13	NULL	NULL	NULL	LDL particles	GP		increased					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_156_s_35	9012651	4 5 6 7 8 9 10 11 12 13 14 15 16 17 18  Furthermore, instead of inducing inhibition, LDL particles increased the binding of fibrinogen to both ADP and proteolytic enzyme - activated platelets.	bind
26233	4	8069	6	13	NULL	NULL	NULL	LDL particles	GP		increased					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_156_s_35	9012651	4 5 6 7 8 9 10 11 12 13 14 15 16 17 18  Furthermore, instead of inducing inhibition, LDL particles increased the binding of fibrinogen to both ADP and proteolytic enzyme - activated platelets.	bind
31750	1	8069	7	NULL	NULL	0	NULL	fibrinogen	NULL		bind	NULL				ADP	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_156_s_35	9012651	4 5 6 7 8 9 10 11 12 13 14 15 16 17 18  Furthermore, instead of inducing inhibition, LDL particles increased the binding of fibrinogen to both ADP and proteolytic enzyme - activated platelets.	bind
31751	2	8069	7	NULL	NULL	0	NULL	fibrinogen	NULL		bind	NULL				 platelets	NULL	proteolytic enzyme - activated			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_156_s_35	9012651	4 5 6 7 8 9 10 11 12 13 14 15 16 17 18  Furthermore, instead of inducing inhibition, LDL particles increased the binding of fibrinogen to both ADP and proteolytic enzyme - activated platelets.	bind
31752	3	8069	7	NULL	NULL	0	NULL	LDL particles	NULL		increase	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_156_s_35	9012651	4 5 6 7 8 9 10 11 12 13 14 15 16 17 18  Furthermore, instead of inducing inhibition, LDL particles increased the binding of fibrinogen to both ADP and proteolytic enzyme - activated platelets.	bind
31753	4	8069	7	NULL	NULL	0	NULL	LDL particles	NULL		increase	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_156_s_35	9012651	4 5 6 7 8 9 10 11 12 13 14 15 16 17 18  Furthermore, instead of inducing inhibition, LDL particles increased the binding of fibrinogen to both ADP and proteolytic enzyme - activated platelets.	bind
26234	1	8070	6	13	NULL	NULL	NULL	Ab	GP		bind		less affinity			p185her2/neu form	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_10_5497_s_46	11320219	4 Ab also binds to the human p185her2/neu form with reduced affinity ( 14).	bind
31754	1	8070	7	NULL	NULL	0	NULL	Ab	NULL		binds	NULL	reduced affinity			p185her2/neu form	NULL	human			NULL		0	NULL	NULL	NULL	gw60_pnas_98_10_5497_s_46	11320219	4 Ab also binds to the human p185her2/neu form with reduced affinity ( 14).	bind
26235	1	8071	6	13	NULL	NULL	NULL	L-canavanine	AminoAcid		bind					eNOS	GP		oxygenase domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_36_25218_s_254	10464242	4 Absence of the  N5 proton and H-bond has been independently described based on an x-ray crystallographic structure of L-canavanine bound to the eNOS oxygenase domain (C. S. Raman, H. Li, P. Martasek, V. Kral, B. S. S. Masters, and T. L. Poulos, submitted for publication).	bind
31757	1	8071	7	NULL	NULL	0	NULL	L-canavanine	NULL		bind	NULL				eNOS	NULL		oxygenase domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_36_25218_s_254	10464242	4 Absence of the  N5 proton and H-bond has been independently described based on an x-ray crystallographic structure of L-canavanine bound to the eNOS oxygenase domain (C. S. Raman, H. Li, P. Martasek, V. Kral, B. S. S. Masters, and T. L. Poulos, submitted for publication).	bind
26236	1	8072	6	13	NULL	NULL	NULL	clathrin	GP	cytosolic	bind		avidly			HIP1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_49_46230_s_201	11577110	4 Although cytosolic clathrin binds avidly to the HIP1 GST fusions, we note that HIP1M1 reproducibly interacts more efficiently with soluble trimers than the HIP1M2 segment.	bind
26237	2	8072	6	13	NULL	NULL	NULL	HIP1M1	GP		interacts with					trimers	GP	soluble			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_49_46230_s_201	11577110	4 Although cytosolic clathrin binds avidly to the HIP1 GST fusions, we note that HIP1M1 reproducibly interacts more efficiently with soluble trimers than the HIP1M2 segment.	bind
26238	3	8072	6	13	NULL	NULL	NULL	HIP1M1	GP		interacts with					HIP1M2 segment	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_49_46230_s_201	11577110	4 Although cytosolic clathrin binds avidly to the HIP1 GST fusions, we note that HIP1M1 reproducibly interacts more efficiently with soluble trimers than the HIP1M2 segment.	bind
26239	4	8072	6	13	NULL	NULL	NULL	statement 2	Process		is more efficient than					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_49_46230_s_201	11577110	4 Although cytosolic clathrin binds avidly to the HIP1 GST fusions, we note that HIP1M1 reproducibly interacts more efficiently with soluble trimers than the HIP1M2 segment.	bind
46542	5	8072	6	13	NULL	NULL	NULL	HIP1	GP		is a type of					GST fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_49_46230_s_201	11577110	4 Although cytosolic clathrin binds avidly to the HIP1 GST fusions, we note that HIP1M1 reproducibly interacts more efficiently with soluble trimers than the HIP1M2 segment.	bind
32059	1	8072	7	10	NULL	0	NULL	clathrin	NULL	cytosolic	binds	NULL	avidly			HIP1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_49_46230_s_201	11577110	4 Although cytosolic clathrin binds avidly to the HIP1 GST fusions, we note that HIP1M1 reproducibly interacts more efficiently with soluble trimers than the HIP1M2 segment.	bind
32060	2	8072	7	NULL	NULL	0	NULL	HIP1M1	NULL		interacts with	NULL	reproducibly			 trimers	NULL	soluble			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_49_46230_s_201	11577110	4 Although cytosolic clathrin binds avidly to the HIP1 GST fusions, we note that HIP1M1 reproducibly interacts more efficiently with soluble trimers than the HIP1M2 segment.	bind
32061	3	8072	7	NULL	NULL	0	NULL	HIP1M1	NULL		interacts with	NULL				HIP1M2 segment	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_49_46230_s_201	11577110	4 Although cytosolic clathrin binds avidly to the HIP1 GST fusions, we note that HIP1M1 reproducibly interacts more efficiently with soluble trimers than the HIP1M2 segment.	bind
32062	4	8072	7	NULL	NULL	0	NULL	statement 2	NULL		is more efficient than	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_49_46230_s_201	11577110	4 Although cytosolic clathrin binds avidly to the HIP1 GST fusions, we note that HIP1M1 reproducibly interacts more efficiently with soluble trimers than the HIP1M2 segment.	bind
46543	5	8072	7	10	NULL	0	NULL	HIP1	NULL		is a type of	NULL				GST fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_49_46230_s_201	11577110	4 Although cytosolic clathrin binds avidly to the HIP1 GST fusions, we note that HIP1M1 reproducibly interacts more efficiently with soluble trimers than the HIP1M2 segment.	bind
26240	1	8073	6	13	NULL	NULL	NULL	CHD3	GP		does not bind							methylated	lysine residues		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_51_41789_s_111	16263726	4 Based on the requirement of the KW xxW motif, it is unlikely that CHD3 or CHD4 bind to methylated lysine residues ( Fig. 3).	bind
26241	2	8073	6	13	NULL	NULL	NULL	CHD4	GP		does not bind							methylated	lysine residues		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_51_41789_s_111	16263726	4 Based on the requirement of the KW xxW motif, it is unlikely that CHD3 or CHD4 bind to methylated lysine residues ( Fig. 3).	bind
26242	3	8073	6	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_51_41789_s_111	16263726	4 Based on the requirement of the KW xxW motif, it is unlikely that CHD3 or CHD4 bind to methylated lysine residues ( Fig. 3).	bind
32063	1	8073	7	10	NULL	0	NULL	CHD3	NULL		does not bind	NULL					NULL	methylated	lysine residues		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_51_41789_s_111	16263726	4 Based on the requirement of the KW xxW motif, it is unlikely that CHD3 or CHD4 bind to methylated lysine residues ( Fig. 3).	bind
32064	2	8073	7	10	NULL	0	NULL	CHD4	NULL		does not bind	NULL					NULL	methylated	lysine residues		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_51_41789_s_111	16263726	4 Based on the requirement of the KW xxW motif, it is unlikely that CHD3 or CHD4 bind to methylated lysine residues ( Fig. 3).	bind
32065	3	8073	7	10	NULL	0	NULL	statement 1			is an alternative to					statement 2					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_51_41789_s_111	16263726	4 Based on the requirement of the KW xxW motif, it is unlikely that CHD3 or CHD4 bind to methylated lysine residues ( Fig. 3).	bind
26243	1	8075	6	13	NULL	NULL	NULL	C7	NucleicAcid		bind					TBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_14623_s_156	11278275	4 C7 binding to TBP in buffer ( light solid line) differs profoundly from that of the consensus sequence, but successively approaches the AdMLP.	bind
32067	1	8075	7	NULL	NULL	0	NULL	 C7	NULL		bind	NULL				TBP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_18_14623_s_156	11278275	4 C7 binding to TBP in buffer ( light solid line) differs profoundly from that of the consensus sequence, but successively approaches the AdMLP.	bind
32072	1	8076	7	13	NULL	NULL	NULL	ERalphaKOCH	Organism	mice	bind		high-affinity			estradiol	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_10_1087_s_118	12039798	4 ERalphaKOCH mice have marked reproductive phenotypes, 4, 12 but also display a low level of residual, high-affinity estradiol binding, as well as expression of two ERalpha-derived transcripts, one of which encodes a truncated ERalpha with intact DNA- and hormone-binding domains.	bind
32079	2	8076	7	13	NULL	NULL	NULL	ERalphaKOCH	Organism	mice	express					ERalpha-derived transcripts	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_10_1087_s_118	12039798	4 ERalphaKOCH mice have marked reproductive phenotypes, 4, 12 but also display a low level of residual, high-affinity estradiol binding, as well as expression of two ERalpha-derived transcripts, one of which encodes a truncated ERalpha with intact DNA- and hormone-binding domains.	bind
32080	3	8076	7	13	NULL	NULL	NULL	ERalpha-derived transcripts	GP		encode					ERalpha	GP	truncated	DNA binding domain		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_10_1087_s_118	12039798	4 ERalphaKOCH mice have marked reproductive phenotypes, 4, 12 but also display a low level of residual, high-affinity estradiol binding, as well as expression of two ERalpha-derived transcripts, one of which encodes a truncated ERalpha with intact DNA- and hormone-binding domains.	bind
32081	4	8076	7	13	NULL	NULL	NULL	ERalpha-derived transcripts	GP		encode					ERalpha	GP		hormone-binding domain		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_10_1087_s_118	12039798	4 ERalphaKOCH mice have marked reproductive phenotypes, 4, 12 but also display a low level of residual, high-affinity estradiol binding, as well as expression of two ERalpha-derived transcripts, one of which encodes a truncated ERalpha with intact DNA- and hormone-binding domains.	bind
26296	1	8077	6	13	NULL	NULL	NULL	AR structures	GP		bind					DHT	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_10_6648_s_489	16365032	4 From our original report ( ), a recent report ( ), and as shown here, the absence of a C-19 methyl group in R1881 allows the Trp-741 and Met-745 side chains to adopt a conformation that differs from previously reported AR structures bound with DHT that has the C-19 methyl ( ,  ).	bind
55826	2	8077	6	13	NULL	NULL	NULL	DHT	Chemical		contains								C-19 methyl group		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_10_6648_s_489	16365032	4 From our original report ( ), a recent report ( ), and as shown here, the absence of a C-19 methyl group in R1881 allows the Trp-741 and Met-745 side chains to adopt a conformation that differs from previously reported AR structures bound with DHT that has the C-19 methyl ( ,  ).	bind
32084	1	8077	7	10	NULL	0	NULL	AR structure			bind					DHT					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_10_6648_s_489	16365032	4 From our original report ( ), a recent report ( ), and as shown here, the absence of a C-19 methyl group in R1881 allows the Trp-741 and Met-745 side chains to adopt a conformation that differs from previously reported AR structures bound with DHT that has the C-19 methyl ( ,  ).	bind
32085	2	8077	7	10	NULL	0	NULL	DHT			contains								C-19 methyl group		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_10_6648_s_489	16365032	4 From our original report ( ), a recent report ( ), and as shown here, the absence of a C-19 methyl group in R1881 allows the Trp-741 and Met-745 side chains to adopt a conformation that differs from previously reported AR structures bound with DHT that has the C-19 methyl ( ,  ).	bind
26244	1	8078	6	13	NULL	NULL	NULL	GST-M-RIP	GP		bind			545-878;; CC2 		MBS	GP	endogenous	leucine zipper domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_51_51484_s_250	14506264	4 GST-M-RIP-(545 - 878) bound both endogenous MBS and GFP-MBS, but failed to bind the GFP-MBSLZ mutant ( Fig. 4 E), supporting further that the M-RIP-MBS interaction is mediated by the CC2 of M-RIP and the leucine zipper domain of MBS.	bind
26245	2	8078	6	13	NULL	NULL	NULL	GST-M-RIP	GP		bind			545-878;; CC2		GFP-MBS	GP		leucine zipper domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_51_51484_s_250	14506264	4 GST-M-RIP-(545 - 878) bound both endogenous MBS and GFP-MBS, but failed to bind the GFP-MBSLZ mutant ( Fig. 4 E), supporting further that the M-RIP-MBS interaction is mediated by the CC2 of M-RIP and the leucine zipper domain of MBS.	bind
26246	3	8078	6	13	NULL	NULL	NULL	GST-M-RIP	GP		does not bind					GFP-MBS	GP	mutant	LZ		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_51_51484_s_250	14506264	4 GST-M-RIP-(545 - 878) bound both endogenous MBS and GFP-MBS, but failed to bind the GFP-MBSLZ mutant ( Fig. 4 E), supporting further that the M-RIP-MBS interaction is mediated by the CC2 of M-RIP and the leucine zipper domain of MBS.	bind
32086	1	8078	7	13	NULL	NULL	NULL	GST-M-RIP	GP		bind			545 - 878		MBS	GP	endogenous			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_51_51484_s_250	14506264	4 GST-M-RIP-(545 - 878) bound both endogenous MBS and GFP-MBS, but failed to bind the GFP-MBSLZ mutant ( Fig. 4 E), supporting further that the M-RIP-MBS interaction is mediated by the CC2 of M-RIP and the leucine zipper domain of MBS.	bind
32087	2	8078	7	NULL	NULL	0	NULL	GST-M-RIP	NULL		bind	NULL		545 - 878		GFP-MBS	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_51_51484_s_250	14506264	4 GST-M-RIP-(545 - 878) bound both endogenous MBS and GFP-MBS, but failed to bind the GFP-MBSLZ mutant ( Fig. 4 E), supporting further that the M-RIP-MBS interaction is mediated by the CC2 of M-RIP and the leucine zipper domain of MBS.	bind
32088	3	8078	7	NULL	NULL	0	NULL	GST-M-RIP	NULL		does not bind	NULL				GFP-MBSLZ	NULL	mutant			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_51_51484_s_250	14506264	4 GST-M-RIP-(545 - 878) bound both endogenous MBS and GFP-MBS, but failed to bind the GFP-MBSLZ mutant ( Fig. 4 E), supporting further that the M-RIP-MBS interaction is mediated by the CC2 of M-RIP and the leucine zipper domain of MBS.	bind
32089	4	8078	7	NULL	NULL	0	NULL	M-RIP 	NULL		mediates	NULL		CC2		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_51_51484_s_250	14506264	4 GST-M-RIP-(545 - 878) bound both endogenous MBS and GFP-MBS, but failed to bind the GFP-MBSLZ mutant ( Fig. 4 E), supporting further that the M-RIP-MBS interaction is mediated by the CC2 of M-RIP and the leucine zipper domain of MBS.	bind
32090	5	8078	7	NULL	NULL	0	NULL	M-RIP 	NULL		mediates	NULL		CC2		statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_51_51484_s_250	14506264	4 GST-M-RIP-(545 - 878) bound both endogenous MBS and GFP-MBS, but failed to bind the GFP-MBSLZ mutant ( Fig. 4 E), supporting further that the M-RIP-MBS interaction is mediated by the CC2 of M-RIP and the leucine zipper domain of MBS.	bind
32091	6	8078	7	NULL	NULL	0	NULL	MBS	NULL		mediates	NULL		leucine zipper domain		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_51_51484_s_250	14506264	4 GST-M-RIP-(545 - 878) bound both endogenous MBS and GFP-MBS, but failed to bind the GFP-MBSLZ mutant ( Fig. 4 E), supporting further that the M-RIP-MBS interaction is mediated by the CC2 of M-RIP and the leucine zipper domain of MBS.	bind
32092	7	8078	7	NULL	NULL	0	NULL	MBS	NULL		mediates	NULL		leucine zipper domain		statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_51_51484_s_250	14506264	4 GST-M-RIP-(545 - 878) bound both endogenous MBS and GFP-MBS, but failed to bind the GFP-MBSLZ mutant ( Fig. 4 E), supporting further that the M-RIP-MBS interaction is mediated by the CC2 of M-RIP and the leucine zipper domain of MBS.	bind
26247	1	8079	6	13	NULL	NULL	NULL	SecY	GP	mutant	bind					SecA	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_10_9097_s_264	15618215	4 However, when tested with mutant SecY(prlA4), which binds SecA with higher affinity ( ), its efficiency reached 74%.	bind
46544	2	8079	6	13	NULL	NULL	NULL	SecY	GP	mutant	is					SecY	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_10_9097_s_264	15618215	4 However, when tested with mutant SecY(prlA4), which binds SecA with higher affinity ( ), its efficiency reached 74%.	bind
32093	1	8079	7	NULL	NULL	0	NULL	 SecY	NULL	mutant	binds	NULL	high affinity			SecA	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_9097_s_264	15618215	4 However, when tested with mutant SecY(prlA4), which binds SecA with higher affinity ( ), its efficiency reached 74%.	bind
32094	2	8079	7	10	NULL	0	NULL	 SecY	NULL	mutant	is	NULL				prlA4	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_10_9097_s_264	15618215	4 However, when tested with mutant SecY(prlA4), which binds SecA with higher affinity ( ), its efficiency reached 74%.	bind
26248	1	8080	6	13	NULL	NULL	NULL	TIMP-4	GP	exogenous	bind					MT1-MMP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_52_41415_s_167	10998420	4 Immunoblot analysis demonstrated the cell association of the exogenous TIMP-4 with ( / )  Timp2 mutant cells expressing MT1-MMP (Fig.  2 C,  lane 2) suggesting the binding of TIMP-4 to MT1-MMP.	bind
46550	2	8080	6	13	NULL	NULL	NULL	Timp2 mutant cells	Cell		express					MT1-MMP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_52_41415_s_167	10998420	4 Immunoblot analysis demonstrated the cell association of the exogenous TIMP-4 with ( / )  Timp2 mutant cells expressing MT1-MMP (Fig.  2 C,  lane 2) suggesting the binding of TIMP-4 to MT1-MMP.	bind
46551	3	8080	6	13	NULL	NULL	NULL	statement 1	Process		occurs in					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_52_41415_s_167	10998420	4 Immunoblot analysis demonstrated the cell association of the exogenous TIMP-4 with ( / )  Timp2 mutant cells expressing MT1-MMP (Fig.  2 C,  lane 2) suggesting the binding of TIMP-4 to MT1-MMP.	bind
32095	1	8080	7	10	NULL	0	NULL	TIMP-4	NULL	exogenous	bind	NULL				MT1-MMP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_52_41415_s_167	10998420	4 Immunoblot analysis demonstrated the cell association of the exogenous TIMP-4 with ( / )  Timp2 mutant cells expressing MT1-MMP (Fig.  2 C,  lane 2) suggesting the binding of TIMP-4 to MT1-MMP.	bind
46552	2	8080	7	10	NULL	0	NULL	Timp2 mutant cells	NULL		express	NULL				MT1-MMP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_52_41415_s_167	10998420	4 Immunoblot analysis demonstrated the cell association of the exogenous TIMP-4 with ( / )  Timp2 mutant cells expressing MT1-MMP (Fig.  2 C,  lane 2) suggesting the binding of TIMP-4 to MT1-MMP.	bind
46553	3	8080	7	10	NULL	0	NULL	statement 1	NULL		occurs in	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_52_41415_s_167	10998420	4 Immunoblot analysis demonstrated the cell association of the exogenous TIMP-4 with ( / )  Timp2 mutant cells expressing MT1-MMP (Fig.  2 C,  lane 2) suggesting the binding of TIMP-4 to MT1-MMP.	bind
26249	1	8081	6	13	NULL	NULL	NULL				does not bind			NP XY motifs		AP-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_18_12751_s_283	16517607	4 In addition, a potential adaptor-binding NP XY motif (N19 PGY) is also present nearby; however, NP XY motifs do not bind to AP-1.	bind
55827	2	8081	6	13	NULL	NULL	NULL	N19 PGY	GP		is					NP XY motif	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_18_12751_s_283	16517607	4 In addition, a potential adaptor-binding NP XY motif (N19 PGY) is also present nearby; however, NP XY motifs do not bind to AP-1.	bind
55828	3	8081	6	13	NULL	NULL	NULL	NP XY motif	GP		is a type of					potential adaptor-binding motif	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_18_12751_s_283	16517607	4 In addition, a potential adaptor-binding NP XY motif (N19 PGY) is also present nearby; however, NP XY motifs do not bind to AP-1.	bind
32096	1	8081	7	NULL	NULL	0	NULL		NULL		does not bind	NULL		NP XY motifs		AP-1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_18_12751_s_283	16517607	4 In addition, a potential adaptor-binding NP XY motif (N19 PGY) is also present nearby; however, NP XY motifs do not bind to AP-1.	bind
32097	2	8081	7	10	NULL	0	NULL	N19 PGY			is					NP XY motif					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_18_12751_s_283	16517607	4 In addition, a potential adaptor-binding NP XY motif (N19 PGY) is also present nearby; however, NP XY motifs do not bind to AP-1.	bind
32098	3	8081	7	10	NULL	0	NULL	NP XY motif			is a type of					potential adaptor-binding motif					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_18_12751_s_283	16517607	4 In addition, a potential adaptor-binding NP XY motif (N19 PGY) is also present nearby; however, NP XY motifs do not bind to AP-1.	bind
26250	1	8082	6	13	NULL	NULL	NULL	Munc-18-1	GP		bind					syntaxins	GP				NULL	neurons	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_48_31633_s_145	9822620	4 In neurons, the X11alpha.mLin-2.mLin-7 protein complexes may bind to specific target membranes sites via Munc-18-1, a protein that can bind syntaxins and possibly modulate trafficking and secretion ( 29).	bind
26251	2	8082	6	13	NULL	NULL	NULL	X11alpha.mLin-2.mLin-7 protein complex	GP		bind		may			target membranes sites	CellComponent	specific			NULL	neurons	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_48_31633_s_145	9822620	4 In neurons, the X11alpha.mLin-2.mLin-7 protein complexes may bind to specific target membranes sites via Munc-18-1, a protein that can bind syntaxins and possibly modulate trafficking and secretion ( 29).	bind
26252	3	8082	6	13	NULL	NULL	NULL	statement 2	Process		occurs via					Munc-18-1	GP				NULL	neurons	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_48_31633_s_145	9822620	4 In neurons, the X11alpha.mLin-2.mLin-7 protein complexes may bind to specific target membranes sites via Munc-18-1, a protein that can bind syntaxins and possibly modulate trafficking and secretion ( 29).	bind
26253	4	8082	6	13	NULL	NULL	NULL	Munc-18-1	GP		modulate		possibly			trafficking	Process				NULL	neurons	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_48_31633_s_145	9822620	4 In neurons, the X11alpha.mLin-2.mLin-7 protein complexes may bind to specific target membranes sites via Munc-18-1, a protein that can bind syntaxins and possibly modulate trafficking and secretion ( 29).	bind
26254	5	8082	6	13	NULL	NULL	NULL	Munc-18-1	GP		modulate		possibly			secretion	Process				NULL	neurons	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_48_31633_s_145	9822620	4 In neurons, the X11alpha.mLin-2.mLin-7 protein complexes may bind to specific target membranes sites via Munc-18-1, a protein that can bind syntaxins and possibly modulate trafficking and secretion ( 29).	bind
32100	1	8082	7	10	NULL	0	NULL	X11alpha.mLin-2.mLin-7 protein complex	NULL		bind	NULL	may			target membranes sites	NULL	specific			NULL	neurons	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_48_31633_s_145	9822620	4 In neurons, the X11alpha.mLin-2.mLin-7 protein complexes may bind to specific target membranes sites via Munc-18-1, a protein that can bind syntaxins and possibly modulate trafficking and secretion ( 29).	bind
32104	2	8082	7	NULL	NULL	0	NULL	statement 1	NULL		occurs via	NULL				Munc-18-1	NULL				NULL	neurons	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_48_31633_s_145	9822620	4 In neurons, the X11alpha.mLin-2.mLin-7 protein complexes may bind to specific target membranes sites via Munc-18-1, a protein that can bind syntaxins and possibly modulate trafficking and secretion ( 29).	bind
32105	3	8082	7	NULL	NULL	0	NULL	Munc-18-1	NULL		bind	NULL				syntaxins	NULL				NULL	neurons	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_48_31633_s_145	9822620	4 In neurons, the X11alpha.mLin-2.mLin-7 protein complexes may bind to specific target membranes sites via Munc-18-1, a protein that can bind syntaxins and possibly modulate trafficking and secretion ( 29).	bind
32107	4	8082	7	10	NULL	0	NULL	statement 3	NULL		modulate	NULL	possibly			trafficking	NULL				NULL	neurons	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_48_31633_s_145	9822620	4 In neurons, the X11alpha.mLin-2.mLin-7 protein complexes may bind to specific target membranes sites via Munc-18-1, a protein that can bind syntaxins and possibly modulate trafficking and secretion ( 29).	bind
32108	5	8082	7	10	NULL	0	NULL	statement 3	NULL		modulate	NULL	possibly			secretion	NULL				NULL	neurons	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_48_31633_s_145	9822620	4 In neurons, the X11alpha.mLin-2.mLin-7 protein complexes may bind to specific target membranes sites via Munc-18-1, a protein that can bind syntaxins and possibly modulate trafficking and secretion ( 29).	bind
26255	1	8083	6	13	NULL	NULL	NULL	GA	Chemical		bind					hsp90	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_38_23843_s_257	9295332	4 Instead, we propose that GA binding to hsp90 locks the chaperone into its ADP-dependent configuration.	bind
26256	2	8083	6	13	NULL	NULL	NULL	hsp90	GP		is a type of					chaperone	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_38_23843_s_257	9295332	4 Instead, we propose that GA binding to hsp90 locks the chaperone into its ADP-dependent configuration.	bind
55829	3	8083	6	13	NULL	NULL	NULL	hsp90	GP		locked into					ADP-dependent configuration	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_38_23843_s_257	9295332	4 Instead, we propose that GA binding to hsp90 locks the chaperone into its ADP-dependent configuration.	bind
55830	4	8083	6	13	NULL	NULL	NULL	statement 1	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_38_23843_s_257	9295332	4 Instead, we propose that GA binding to hsp90 locks the chaperone into its ADP-dependent configuration.	bind
32113	1	8083	7	NULL	NULL	0	NULL	GA	NULL		bind	NULL				hsp90	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_38_23843_s_257	9295332	4 Instead, we propose that GA binding to hsp90 locks the chaperone into its ADP-dependent configuration.	bind
32114	2	8083	7	10	NULL	0	NULL	hsp90			is a type of					chaperone					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_38_23843_s_257	9295332	4 Instead, we propose that GA binding to hsp90 locks the chaperone into its ADP-dependent configuration.	bind
32115	3	8083	7	10	NULL	0	NULL	hsp90			locked into					ADP-dependent configuration					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_38_23843_s_257	9295332	4 Instead, we propose that GA binding to hsp90 locks the chaperone into its ADP-dependent configuration.	bind
55831	4	8083	7	10	NULL	0	NULL	statement 1			leads to					statement 3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_38_23843_s_257	9295332	4 Instead, we propose that GA binding to hsp90 locks the chaperone into its ADP-dependent configuration.	bind
26297	1	8084	6	13	NULL	NULL	NULL	ADP	Chemical		bind					Hsp70	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_35_22506_s_293	9712876	4 Interestingly, BAG-1 and Hip regulate Hsp70 activity in opposite manners: Hip stabilizes the ADP-bound form of Hsp70, promoting formation with target peptides ( 50), while BAG-1 stimulates the release of ADP and peptide substrates ( 21).	bind
26298	2	8084	6	13	NULL	NULL	NULL	Hip	GP		stabilizes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_35_22506_s_293	9712876	4 Interestingly, BAG-1 and Hip regulate Hsp70 activity in opposite manners: Hip stabilizes the ADP-bound form of Hsp70, promoting formation with target peptides ( 50), while BAG-1 stimulates the release of ADP and peptide substrates ( 21).	bind
26299	3	8084	6	13	NULL	NULL	NULL	BAG-1	GP		stimulates					ADP	Chemical	release of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_35_22506_s_293	9712876	4 Interestingly, BAG-1 and Hip regulate Hsp70 activity in opposite manners: Hip stabilizes the ADP-bound form of Hsp70, promoting formation with target peptides ( 50), while BAG-1 stimulates the release of ADP and peptide substrates ( 21).	bind
26300	4	8084	6	13	NULL	NULL	NULL	BAG-1	GP		stimulates					peptide substrates	GP	release of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_35_22506_s_293	9712876	4 Interestingly, BAG-1 and Hip regulate Hsp70 activity in opposite manners: Hip stabilizes the ADP-bound form of Hsp70, promoting formation with target peptides ( 50), while BAG-1 stimulates the release of ADP and peptide substrates ( 21).	bind
32116	1	8084	7	NULL	NULL	0	NULL	ADP	NULL		bind	NULL				Hsp70	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_35_22506_s_293	9712876	4 Interestingly, BAG-1 and Hip regulate Hsp70 activity in opposite manners: Hip stabilizes the ADP-bound form of Hsp70, promoting formation with target peptides ( 50), while BAG-1 stimulates the release of ADP and peptide substrates ( 21).	bind
32117	2	8084	7	NULL	NULL	0	NULL	Hip	NULL		stabilizes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_35_22506_s_293	9712876	4 Interestingly, BAG-1 and Hip regulate Hsp70 activity in opposite manners: Hip stabilizes the ADP-bound form of Hsp70, promoting formation with target peptides ( 50), while BAG-1 stimulates the release of ADP and peptide substrates ( 21).	bind
32118	3	8084	7	NULL	NULL	0	NULL	statement 2	NULL		promotes	NULL				target peptides	NULL	formation with			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_35_22506_s_293	9712876	4 Interestingly, BAG-1 and Hip regulate Hsp70 activity in opposite manners: Hip stabilizes the ADP-bound form of Hsp70, promoting formation with target peptides ( 50), while BAG-1 stimulates the release of ADP and peptide substrates ( 21).	bind
32119	4	8084	7	NULL	NULL	0	NULL	BAG-1 	NULL		stimulate	NULL				ADP	NULL	release of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_35_22506_s_293	9712876	4 Interestingly, BAG-1 and Hip regulate Hsp70 activity in opposite manners: Hip stabilizes the ADP-bound form of Hsp70, promoting formation with target peptides ( 50), while BAG-1 stimulates the release of ADP and peptide substrates ( 21).	bind
32120	5	8084	7	NULL	NULL	0	NULL	BAG-1 	NULL		stimulates	NULL				peptide substrates	NULL	release of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_35_22506_s_293	9712876	4 Interestingly, BAG-1 and Hip regulate Hsp70 activity in opposite manners: Hip stabilizes the ADP-bound form of Hsp70, promoting formation with target peptides ( 50), while BAG-1 stimulates the release of ADP and peptide substrates ( 21).	bind
32121	6	8084	7	NULL	NULL	0	NULL	BAG-1 	NULL		regulate	NULL				Hsp70	NULL	activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_35_22506_s_293	9712876	4 Interestingly, BAG-1 and Hip regulate Hsp70 activity in opposite manners: Hip stabilizes the ADP-bound form of Hsp70, promoting formation with target peptides ( 50), while BAG-1 stimulates the release of ADP and peptide substrates ( 21).	bind
32122	7	8084	7	NULL	NULL	0	NULL	Hip	NULL		regulate	NULL				Hsp70	NULL	activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_35_22506_s_293	9712876	4 Interestingly, BAG-1 and Hip regulate Hsp70 activity in opposite manners: Hip stabilizes the ADP-bound form of Hsp70, promoting formation with target peptides ( 50), while BAG-1 stimulates the release of ADP and peptide substrates ( 21).	bind
32123	8	8084	7	NULL	NULL	0	NULL	statement 6 	NULL		is in opposite way to	NULL				statement 7	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_35_22506_s_293	9712876	4 Interestingly, BAG-1 and Hip regulate Hsp70 activity in opposite manners: Hip stabilizes the ADP-bound form of Hsp70, promoting formation with target peptides ( 50), while BAG-1 stimulates the release of ADP and peptide substrates ( 21).	bind
26301	1	8085	6	13	NULL	NULL	NULL				bind			E191A		DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_16_14306_s_194	11827971	4 It is important to note that E191A, E233A, and K235A show largely unaltered DNA binding and cleavage activity.	bind
26302	2	8085	6	13	NULL	NULL	NULL				exhibits			E191A		clevage activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_16_14306_s_194	11827971	4 It is important to note that E191A, E233A, and K235A show largely unaltered DNA binding and cleavage activity.	bind
26303	3	8085	6	13	NULL	NULL	NULL				bind			E233A		DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_16_14306_s_194	11827971	4 It is important to note that E191A, E233A, and K235A show largely unaltered DNA binding and cleavage activity.	bind
26304	4	8085	6	13	NULL	NULL	NULL				exhibits			E233A		clevage activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_16_14306_s_194	11827971	4 It is important to note that E191A, E233A, and K235A show largely unaltered DNA binding and cleavage activity.	bind
26305	5	8085	6	13	NULL	NULL	NULL				bind			K235A		DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_16_14306_s_194	11827971	4 It is important to note that E191A, E233A, and K235A show largely unaltered DNA binding and cleavage activity.	bind
26306	6	8085	6	13	NULL	NULL	NULL				exhibits			K235A		clevage activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_16_14306_s_194	11827971	4 It is important to note that E191A, E233A, and K235A show largely unaltered DNA binding and cleavage activity.	bind
26307	1	8086	6	13	NULL	NULL	NULL	apo A-I	GP		is abundant on					HDL3-E	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1333_s_178	12089072	4 It may be that apo A-I, which is abundant on HDL3-E, interacts with non-proteoglycan ECM components, because previous studies have shown that apo A-I can bind fibronectin and collagen, for example.	bind
26308	2	8086	6	13	NULL	NULL	NULL	apo A-I	GP		interacts with					ECM components	CellComponent	non-proteoglycan			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1333_s_178	12089072	4 It may be that apo A-I, which is abundant on HDL3-E, interacts with non-proteoglycan ECM components, because previous studies have shown that apo A-I can bind fibronectin and collagen, for example.	bind
26309	3	8086	6	13	NULL	NULL	NULL	apo A-I	GP		bind					fibrinogen	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1333_s_178	12089072	4 It may be that apo A-I, which is abundant on HDL3-E, interacts with non-proteoglycan ECM components, because previous studies have shown that apo A-I can bind fibronectin and collagen, for example.	bind
26310	4	8086	6	13	NULL	NULL	NULL	apo A-I	GP		bind					collagen	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1333_s_178	12089072	4 It may be that apo A-I, which is abundant on HDL3-E, interacts with non-proteoglycan ECM components, because previous studies have shown that apo A-I can bind fibronectin and collagen, for example.	bind
32130	1	8086	7	10	NULL	0	NULL	apo A-I			interacts with					ECM components		non-proteoglycan			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1333_s_178	12089072	4 It may be that apo A-I, which is abundant on HDL3-E, interacts with non-proteoglycan ECM components, because previous studies have shown that apo A-I can bind fibronectin and collagen, for example.	bind
32131	2	8086	7	NULL	NULL	0	NULL	apo A-I 	NULL		bind	NULL				fibronectin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_12_1333_s_178	12089072	4 It may be that apo A-I, which is abundant on HDL3-E, interacts with non-proteoglycan ECM components, because previous studies have shown that apo A-I can bind fibronectin and collagen, for example.	bind
32132	3	8086	7	NULL	NULL	0	NULL	apo A-I	NULL		bind	NULL				collagen	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1333_s_178	12089072	4 It may be that apo A-I, which is abundant on HDL3-E, interacts with non-proteoglycan ECM components, because previous studies have shown that apo A-I can bind fibronectin and collagen, for example.	bind
32133	4	8086	7	NULL	NULL	0	NULL	apo A-I	NULL		is abundant on	NULL				HDL3-E	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_12_1333_s_178	12089072	4 It may be that apo A-I, which is abundant on HDL3-E, interacts with non-proteoglycan ECM components, because previous studies have shown that apo A-I can bind fibronectin and collagen, for example.	bind
26311	1	8087	6	13	NULL	NULL	NULL	CCR2	GP		is					CC chemokine receptor 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_2_244_s_26	12588766	4 MCP-1 specifically binds to CC chemokine receptor 2 (CCR2) and fulfills its function.	bind
26312	2	8087	6	13	NULL	NULL	NULL	MCP-1	GP		bind		specifically			CCR2	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_2_244_s_26	12588766	4 MCP-1 specifically binds to CC chemokine receptor 2 (CCR2) and fulfills its function.	bind
32135	1	8087	7	NULL	NULL	0	NULL	MCP-1	NULL		binds	NULL	specifically			CCR2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_2_244_s_26	12588766	4 MCP-1 specifically binds to CC chemokine receptor 2 (CCR2) and fulfills its function.	bind
32136	2	8087	7	10	NULL	0	NULL	CCR2			is					CC chemokine receptor 2					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_2_244_s_26	12588766	4 MCP-1 specifically binds to CC chemokine receptor 2 (CCR2) and fulfills its function.	bind
26313	1	8089	6	13	NULL	NULL	NULL	CCR2	GP		is					CC chemokine receptor 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_864_s_21	15016641	4 Monocytes express CC chemokine receptor 2 (CCR2), which binds monocyte chemoattractant protein-1 (MCP-1), leading to beta integrin-mediated firm adhesion and subsequent transmigration of adhered monocytes through the vascular endothelium.	bind
26314	2	8089	6	13	NULL	NULL	NULL	MCP-1	GP		is					monocyte chemoattractant protein-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_864_s_21	15016641	4 Monocytes express CC chemokine receptor 2 (CCR2), which binds monocyte chemoattractant protein-1 (MCP-1), leading to beta integrin-mediated firm adhesion and subsequent transmigration of adhered monocytes through the vascular endothelium.	bind
26315	3	8089	6	13	NULL	NULL	NULL	monocytes	Cell		express					CCR2 	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_864_s_21	15016641	4 Monocytes express CC chemokine receptor 2 (CCR2), which binds monocyte chemoattractant protein-1 (MCP-1), leading to beta integrin-mediated firm adhesion and subsequent transmigration of adhered monocytes through the vascular endothelium.	bind
26316	4	8089	6	13	NULL	NULL	NULL	statement 3	GP		bind					MCP-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_864_s_21	15016641	4 Monocytes express CC chemokine receptor 2 (CCR2), which binds monocyte chemoattractant protein-1 (MCP-1), leading to beta integrin-mediated firm adhesion and subsequent transmigration of adhered monocytes through the vascular endothelium.	bind
26317	5	8089	6	13	NULL	NULL	NULL	beta integrin	GP		mediates					firm adhesion	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_864_s_21	15016641	4 Monocytes express CC chemokine receptor 2 (CCR2), which binds monocyte chemoattractant protein-1 (MCP-1), leading to beta integrin-mediated firm adhesion and subsequent transmigration of adhered monocytes through the vascular endothelium.	bind
26318	6	8089	6	13	NULL	NULL	NULL	statement 4	Process		leads to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_864_s_21	15016641	4 Monocytes express CC chemokine receptor 2 (CCR2), which binds monocyte chemoattractant protein-1 (MCP-1), leading to beta integrin-mediated firm adhesion and subsequent transmigration of adhered monocytes through the vascular endothelium.	bind
26319	7	8089	6	13	NULL	NULL	NULL	monocytes	Cell	adhered	migrate through					vascular endothelium	Cell				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_864_s_21	15016641	4 Monocytes express CC chemokine receptor 2 (CCR2), which binds monocyte chemoattractant protein-1 (MCP-1), leading to beta integrin-mediated firm adhesion and subsequent transmigration of adhered monocytes through the vascular endothelium.	bind
26320	8	8089	6	13	NULL	NULL	NULL	statement 4	Process		leads to					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_864_s_21	15016641	4 Monocytes express CC chemokine receptor 2 (CCR2), which binds monocyte chemoattractant protein-1 (MCP-1), leading to beta integrin-mediated firm adhesion and subsequent transmigration of adhered monocytes through the vascular endothelium.	bind
32137	1	8089	7	10	NULL	0	NULL	statement 8	NULL		binds	NULL				MCP-1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_864_s_21	15016641	4 Monocytes express CC chemokine receptor 2 (CCR2), which binds monocyte chemoattractant protein-1 (MCP-1), leading to beta integrin-mediated firm adhesion and subsequent transmigration of adhered monocytes through the vascular endothelium.	bind
32138	2	8089	7	10	NULL	0	NULL	beta integrin	NULL		mediates	NULL				firm adhesion	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_864_s_21	15016641	4 Monocytes express CC chemokine receptor 2 (CCR2), which binds monocyte chemoattractant protein-1 (MCP-1), leading to beta integrin-mediated firm adhesion and subsequent transmigration of adhered monocytes through the vascular endothelium.	bind
32139	3	8089	7	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_864_s_21	15016641	4 Monocytes express CC chemokine receptor 2 (CCR2), which binds monocyte chemoattractant protein-1 (MCP-1), leading to beta integrin-mediated firm adhesion and subsequent transmigration of adhered monocytes through the vascular endothelium.	bind
32140	4	8089	7	10	NULL	0	NULL	monocytes		adhered	migrates through					vascular endothelium					NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_864_s_21	15016641	4 Monocytes express CC chemokine receptor 2 (CCR2), which binds monocyte chemoattractant protein-1 (MCP-1), leading to beta integrin-mediated firm adhesion and subsequent transmigration of adhered monocytes through the vascular endothelium.	bind
32141	5	8089	7	10	NULL	0	NULL	statement 1			leads to					statement 4					NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_864_s_21	15016641	4 Monocytes express CC chemokine receptor 2 (CCR2), which binds monocyte chemoattractant protein-1 (MCP-1), leading to beta integrin-mediated firm adhesion and subsequent transmigration of adhered monocytes through the vascular endothelium.	bind
32142	6	8089	7	NULL	NULL	0	NULL	CCR2	NULL		is	NULL				CC chemokine receptor 2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_864_s_21	15016641	4 Monocytes express CC chemokine receptor 2 (CCR2), which binds monocyte chemoattractant protein-1 (MCP-1), leading to beta integrin-mediated firm adhesion and subsequent transmigration of adhered monocytes through the vascular endothelium.	bind
32143	7	8089	7	NULL	NULL	0	NULL	MCP-1	NULL		is	NULL				monocyte chemoattractant protein-1 	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_864_s_21	15016641	4 Monocytes express CC chemokine receptor 2 (CCR2), which binds monocyte chemoattractant protein-1 (MCP-1), leading to beta integrin-mediated firm adhesion and subsequent transmigration of adhered monocytes through the vascular endothelium.	bind
46564	8	8089	7	10	NULL	0	NULL	monocytes	NULL		express	NULL				CCR2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_864_s_21	15016641	4 Monocytes express CC chemokine receptor 2 (CCR2), which binds monocyte chemoattractant protein-1 (MCP-1), leading to beta integrin-mediated firm adhesion and subsequent transmigration of adhered monocytes through the vascular endothelium.	bind
26767	1	8090	6	13	NULL	NULL	NULL	Tpr-Met protein	GP	wild type	bind					Grb2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_13116_s_154	8662733	4 Moreover, the Tpr-Met mutants that were unable to bind Shc or Grb2 were impaired in their ability to activate the  c-fos promoter compared with the wild-type or Y482F Tpr-Met proteins, which bind to both Grb2 and Shc.	bind
26768	2	8090	6	13	NULL	NULL	NULL	Tpr-Met protein	GP		bind			Y482F		Grb2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_13116_s_154	8662733	4 Moreover, the Tpr-Met mutants that were unable to bind Shc or Grb2 were impaired in their ability to activate the  c-fos promoter compared with the wild-type or Y482F Tpr-Met proteins, which bind to both Grb2 and Shc.	bind
26769	3	8090	6	13	NULL	NULL	NULL	Tpr-Met protein	GP	wild type	bind					Shc	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_13116_s_154	8662733	4 Moreover, the Tpr-Met mutants that were unable to bind Shc or Grb2 were impaired in their ability to activate the  c-fos promoter compared with the wild-type or Y482F Tpr-Met proteins, which bind to both Grb2 and Shc.	bind
26770	4	8090	6	13	NULL	NULL	NULL	Tpr-Met protein	GP		bind			Y482F		Shc	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_13116_s_154	8662733	4 Moreover, the Tpr-Met mutants that were unable to bind Shc or Grb2 were impaired in their ability to activate the  c-fos promoter compared with the wild-type or Y482F Tpr-Met proteins, which bind to both Grb2 and Shc.	bind
26771	5	8090	6	13	NULL	NULL	NULL	Tpr-Met protein	GP	mutant	does not bind					Grb2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_13116_s_154	8662733	4 Moreover, the Tpr-Met mutants that were unable to bind Shc or Grb2 were impaired in their ability to activate the  c-fos promoter compared with the wild-type or Y482F Tpr-Met proteins, which bind to both Grb2 and Shc.	bind
26772	6	8090	6	13	NULL	NULL	NULL	Tpr-Met protein	GP	mutant	does not bind					Shc	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_13116_s_154	8662733	4 Moreover, the Tpr-Met mutants that were unable to bind Shc or Grb2 were impaired in their ability to activate the  c-fos promoter compared with the wild-type or Y482F Tpr-Met proteins, which bind to both Grb2 and Shc.	bind
26773	7	8090	6	13	NULL	NULL	NULL	Tpr-Met protein	GP		activates					c-fos	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_13116_s_154	8662733	4 Moreover, the Tpr-Met mutants that were unable to bind Shc or Grb2 were impaired in their ability to activate the  c-fos promoter compared with the wild-type or Y482F Tpr-Met proteins, which bind to both Grb2 and Shc.	bind
26774	8	8090	6	13	NULL	NULL	NULL	Tpr-Met protein	GP	mutant	does not activate					c-fos	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_13116_s_154	8662733	4 Moreover, the Tpr-Met mutants that were unable to bind Shc or Grb2 were impaired in their ability to activate the  c-fos promoter compared with the wild-type or Y482F Tpr-Met proteins, which bind to both Grb2 and Shc.	bind
32144	1	8090	7	NULL	NULL	0	NULL	Tpr-Met	NULL	mutant	does not bind	NULL					NULL		Shc		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_22_13116_s_154	8662733	4 Moreover, the Tpr-Met mutants that were unable to bind Shc or Grb2 were impaired in their ability to activate the  c-fos promoter compared with the wild-type or Y482F Tpr-Met proteins, which bind to both Grb2 and Shc.	bind
32145	2	8090	7	NULL	NULL	0	NULL	Tpr-Met	NULL	mutant	does not bind	NULL					NULL		Grb2		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_22_13116_s_154	8662733	4 Moreover, the Tpr-Met mutants that were unable to bind Shc or Grb2 were impaired in their ability to activate the  c-fos promoter compared with the wild-type or Y482F Tpr-Met proteins, which bind to both Grb2 and Shc.	bind
32146	3	8090	7	NULL	NULL	0	NULL	statement 1	NULL		is impaired	NULL				c-fos	NULL	to activate		promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_22_13116_s_154	8662733	4 Moreover, the Tpr-Met mutants that were unable to bind Shc or Grb2 were impaired in their ability to activate the  c-fos promoter compared with the wild-type or Y482F Tpr-Met proteins, which bind to both Grb2 and Shc.	bind
32147	4	8090	7	NULL	NULL	0	NULL	Tpr-Met proteins	NULL	wild-type	bind	NULL					NULL		Shc		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_22_13116_s_154	8662733	4 Moreover, the Tpr-Met mutants that were unable to bind Shc or Grb2 were impaired in their ability to activate the  c-fos promoter compared with the wild-type or Y482F Tpr-Met proteins, which bind to both Grb2 and Shc.	bind
32148	5	8090	7	NULL	NULL	0	NULL	Tpr-Met proteins	NULL	wild-type	bind	NULL					NULL		Grb2		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_22_13116_s_154	8662733	4 Moreover, the Tpr-Met mutants that were unable to bind Shc or Grb2 were impaired in their ability to activate the  c-fos promoter compared with the wild-type or Y482F Tpr-Met proteins, which bind to both Grb2 and Shc.	bind
32149	6	8090	7	NULL	NULL	0	NULL	Tpr-Met proteins	NULL		bind	NULL		 Y482F 			NULL		Shc		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_22_13116_s_154	8662733	4 Moreover, the Tpr-Met mutants that were unable to bind Shc or Grb2 were impaired in their ability to activate the  c-fos promoter compared with the wild-type or Y482F Tpr-Met proteins, which bind to both Grb2 and Shc.	bind
32150	7	8090	7	NULL	NULL	0	NULL	Tpr-Met proteins	NULL		bind	NULL		Y482F			NULL		Grb2		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_22_13116_s_154	8662733	4 Moreover, the Tpr-Met mutants that were unable to bind Shc or Grb2 were impaired in their ability to activate the  c-fos promoter compared with the wild-type or Y482F Tpr-Met proteins, which bind to both Grb2 and Shc.	bind
32151	8	8090	7	NULL	NULL	0	NULL	statement 2	NULL		is impaired	NULL				c-fos	NULL	to activate		promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_22_13116_s_154	8662733	4 Moreover, the Tpr-Met mutants that were unable to bind Shc or Grb2 were impaired in their ability to activate the  c-fos promoter compared with the wild-type or Y482F Tpr-Met proteins, which bind to both Grb2 and Shc.	bind
26322	1	8091	6	13	NULL	NULL	NULL	GIPC	GP		bind					type III receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_24627_s_268	11323414	4 Mutating the Class I PDZ binding motif of the type III receptor abolishes binding of GIPC to the type III receptor, but does not effect the interaction between the type III receptor and the type II receptor studied here, establishing that this protein is not an adaptor protein in this interaction.	bind
26323	2	8091	6	13	NULL	NULL	NULL	type III receptor	GP	mutant	abolishes			Class I PDZ binding motif		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_24627_s_268	11323414	4 Mutating the Class I PDZ binding motif of the type III receptor abolishes binding of GIPC to the type III receptor, but does not effect the interaction between the type III receptor and the type II receptor studied here, establishing that this protein is not an adaptor protein in this interaction.	bind
26324	3	8091	6	13	NULL	NULL	NULL	type III receptor	GP		interacts with					type II receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_24627_s_268	11323414	4 Mutating the Class I PDZ binding motif of the type III receptor abolishes binding of GIPC to the type III receptor, but does not effect the interaction between the type III receptor and the type II receptor studied here, establishing that this protein is not an adaptor protein in this interaction.	bind
26325	4	8091	6	13	NULL	NULL	NULL	type III receptor	GP	mutant	has no effect on			Class I PDZ binding motif		statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_24627_s_268	11323414	4 Mutating the Class I PDZ binding motif of the type III receptor abolishes binding of GIPC to the type III receptor, but does not effect the interaction between the type III receptor and the type II receptor studied here, establishing that this protein is not an adaptor protein in this interaction.	bind
32156	1	8091	7	NULL	NULL	0	NULL	GIPC	NULL		bind	NULL				type III receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_27_24627_s_268	11323414	4 Mutating the Class I PDZ binding motif of the type III receptor abolishes binding of GIPC to the type III receptor, but does not effect the interaction between the type III receptor and the type II receptor studied here, establishing that this protein is not an adaptor protein in this interaction.	bind
32157	2	8091	7	NULL	NULL	0	NULL	Type III receptor	NULL	mutant	abolishes	NULL		Class I PDZ binding motif		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_24627_s_268	11323414	4 Mutating the Class I PDZ binding motif of the type III receptor abolishes binding of GIPC to the type III receptor, but does not effect the interaction between the type III receptor and the type II receptor studied here, establishing that this protein is not an adaptor protein in this interaction.	bind
32158	3	8091	7	NULL	NULL	0	NULL	type III receptor	NULL		interacts with	NULL				type II receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_27_24627_s_268	11323414	4 Mutating the Class I PDZ binding motif of the type III receptor abolishes binding of GIPC to the type III receptor, but does not effect the interaction between the type III receptor and the type II receptor studied here, establishing that this protein is not an adaptor protein in this interaction.	bind
32159	4	8091	7	NULL	NULL	0	NULL	Type III receptor	NULL	mutant	does not affect	NULL		Class I PDZ binding motif		statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_27_24627_s_268	11323414	4 Mutating the Class I PDZ binding motif of the type III receptor abolishes binding of GIPC to the type III receptor, but does not effect the interaction between the type III receptor and the type II receptor studied here, establishing that this protein is not an adaptor protein in this interaction.	bind
26775	1	8092	6	13	NULL	NULL	NULL	zonadhesin	GP		bind					ZP	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_41502_s_287	11526117	4 Our detection of differences in ZP binding activity among the various zonadhesin forms suggests that the heterogeneous processing of this protein is functionally important, just as proteolytic activation and heterogeneous multimerization are important for the proper function of vWF ( 10).	bind
26776	2	8092	6	13	NULL	NULL	NULL	zonadhesin	GP	heterogeneous processing of	is important for					zonadhesin	GP	proper function of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_41502_s_287	11526117	4 Our detection of differences in ZP binding activity among the various zonadhesin forms suggests that the heterogeneous processing of this protein is functionally important, just as proteolytic activation and heterogeneous multimerization are important for the proper function of vWF ( 10).	bind
26777	3	8092	6	13	NULL	NULL	NULL	vWF	GP	proteolytic activation of	is important for					vWF	GP	proper function of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_41502_s_287	11526117	4 Our detection of differences in ZP binding activity among the various zonadhesin forms suggests that the heterogeneous processing of this protein is functionally important, just as proteolytic activation and heterogeneous multimerization are important for the proper function of vWF ( 10).	bind
26778	4	8092	6	13	NULL	NULL	NULL	vWF	GP	heterogeneous multimerization of	is important for					vWF	GP	proper function of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_41502_s_287	11526117	4 Our detection of differences in ZP binding activity among the various zonadhesin forms suggests that the heterogeneous processing of this protein is functionally important, just as proteolytic activation and heterogeneous multimerization are important for the proper function of vWF ( 10).	bind
32161	1	8092	7	NULL	NULL	0	NULL	ZP	NULL		binds	NULL				zonadhesin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_44_41502_s_287	11526117	4 Our detection of differences in ZP binding activity among the various zonadhesin forms suggests that the heterogeneous processing of this protein is functionally important, just as proteolytic activation and heterogeneous multimerization are important for the proper function of vWF ( 10).	bind
32162	2	8092	7	NULL	NULL	0	NULL	statement 1	NULL	different binding  activity of	suggests	NULL				zonadhesin	NULL	heterogeneous processing of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_44_41502_s_287	11526117	4 Our detection of differences in ZP binding activity among the various zonadhesin forms suggests that the heterogeneous processing of this protein is functionally important, just as proteolytic activation and heterogeneous multimerization are important for the proper function of vWF ( 10).	bind
32163	3	8092	7	NULL	NULL	0	NULL	vWF	NULL	proteolytic activation	is important for	NULL				vWF	NULL	function of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_44_41502_s_287	11526117	4 Our detection of differences in ZP binding activity among the various zonadhesin forms suggests that the heterogeneous processing of this protein is functionally important, just as proteolytic activation and heterogeneous multimerization are important for the proper function of vWF ( 10).	bind
32164	4	8092	7	NULL	NULL	0	NULL	vWF	NULL	heterogeneous multimerization of	is important for	NULL				vWF	NULL	function of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_44_41502_s_287	11526117	4 Our detection of differences in ZP binding activity among the various zonadhesin forms suggests that the heterogeneous processing of this protein is functionally important, just as proteolytic activation and heterogeneous multimerization are important for the proper function of vWF ( 10).	bind
26328	1	8094	6	13	NULL	NULL	NULL	Galectin-3	GP	purified;;rat	bind					bone acidic glycoprotein-75	GP	isolated			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_21_18840_s_306	11886849	4 Recent quantitative studies show that purified rat galectin-3 binds as well to isolated bone acidic glycoprotein-75 as to monoclonal anti-DNP IgE, the commonly used standard ligand for this receptor.	bind
26329	2	8094	6	13	NULL	NULL	NULL	Galectin-3	GP	purified;;rat	bind					anti-DNP IgE	GP	monoclonal			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_21_18840_s_306	11886849	4 Recent quantitative studies show that purified rat galectin-3 binds as well to isolated bone acidic glycoprotein-75 as to monoclonal anti-DNP IgE, the commonly used standard ligand for this receptor.	bind
32172	1	8094	7	10	NULL	0	NULL	 galectin-3	NULL	purified;;rat	binds	NULL				bone acidic glycoprotein-75	NULL	 isolated			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_21_18840_s_306	11886849	4 Recent quantitative studies show that purified rat galectin-3 binds as well to isolated bone acidic glycoprotein-75 as to monoclonal anti-DNP IgE, the commonly used standard ligand for this receptor.	bind
32173	2	8094	7	10	NULL	0	NULL	galectin-3	NULL	purified;;rat	binds	NULL				anti-DNP IgE	NULL	monoclonal 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_21_18840_s_306	11886849	4 Recent quantitative studies show that purified rat galectin-3 binds as well to isolated bone acidic glycoprotein-75 as to monoclonal anti-DNP IgE, the commonly used standard ligand for this receptor.	bind
26330	1	8095	6	13	NULL	NULL	NULL	GTP	Chemical		bind					ARF3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_18_13465_s_120	10788460	4 Sat1delta5 (8 muM) failed to promote enhanced GTP binding to ARF3 (data not shown) despite its ability to bind to mammalian ARFs.	bind
26331	2	8095	6	13	NULL	NULL	NULL	Sat1delta5	GP		failed to promote					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_18_13465_s_120	10788460	4 Sat1delta5 (8 muM) failed to promote enhanced GTP binding to ARF3 (data not shown) despite its ability to bind to mammalian ARFs.	bind
26332	3	8095	6	13	NULL	NULL	NULL	GTP	Chemical		bind					ARF	GP	mammalian			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_18_13465_s_120	10788460	4 Sat1delta5 (8 muM) failed to promote enhanced GTP binding to ARF3 (data not shown) despite its ability to bind to mammalian ARFs.	bind
32174	1	8095	7	NULL	NULL	0	NULL	GTP	NULL		bind	NULL	enhanced			ARF3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_18_13465_s_120	10788460	4 Sat1delta5 (8 muM) failed to promote enhanced GTP binding to ARF3 (data not shown) despite its ability to bind to mammalian ARFs.	bind
32175	2	8095	7	NULL	NULL	0	NULL	Sat1delta5	NULL		does not promote	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13465_s_120	10788460	4 Sat1delta5 (8 muM) failed to promote enhanced GTP binding to ARF3 (data not shown) despite its ability to bind to mammalian ARFs.	bind
32176	3	8095	7	NULL	NULL	0	NULL	GTP 	NULL		bind	NULL				ARFs	NULL	mammalian			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13465_s_120	10788460	4 Sat1delta5 (8 muM) failed to promote enhanced GTP binding to ARF3 (data not shown) despite its ability to bind to mammalian ARFs.	bind
26333	1	8096	6	13	NULL	NULL	NULL	cTnI	GP	phosphorylated	bind					cTnC	GP		COOH-terminal domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_24_16681_s_63	10358006	4 Taken together, these results allow us to propose that both nonphosphorylated and phosphorylated forms of cTnI bind to the COOH-terminal domain of cTnC with the nonphosphorylated form making limited contacts with the NH2-terminal domain of cTnC.	bind
26334	2	8096	6	13	NULL	NULL	NULL	cTnI	GP	nonphosphorylated	bind					cTnC	GP		COOH-terminal domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_24_16681_s_63	10358006	4 Taken together, these results allow us to propose that both nonphosphorylated and phosphorylated forms of cTnI bind to the COOH-terminal domain of cTnC with the nonphosphorylated form making limited contacts with the NH2-terminal domain of cTnC.	bind
26335	3	8096	6	13	NULL	NULL	NULL	cTnI	GP	nonphosphorylated	contacts with		limited			cTnC	GP		NH2 terminus		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_24_16681_s_63	10358006	4 Taken together, these results allow us to propose that both nonphosphorylated and phosphorylated forms of cTnI bind to the COOH-terminal domain of cTnC with the nonphosphorylated form making limited contacts with the NH2-terminal domain of cTnC.	bind
32177	1	8096	7	10	NULL	0	NULL	cTnI	NULL	nonphosphorylated	binds to	NULL				cTnC	NULL		COOH-terminal domain of		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_24_16681_s_63	10358006	4 Taken together, these results allow us to propose that both nonphosphorylated and phosphorylated forms of cTnI bind to the COOH-terminal domain of cTnC with the nonphosphorylated form making limited contacts with the NH2-terminal domain of cTnC.	bind
32178	2	8096	7	10	NULL	0	NULL	cTnI	NULL	phosphorylated	binds to	NULL				cTnC	NULL		COOH-terminal domain 		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_24_16681_s_63	10358006	4 Taken together, these results allow us to propose that both nonphosphorylated and phosphorylated forms of cTnI bind to the COOH-terminal domain of cTnC with the nonphosphorylated form making limited contacts with the NH2-terminal domain of cTnC.	bind
32179	3	8096	7	10	NULL	0	NULL	cTnI	NULL	nonphosphorylated	 contacts with	NULL	limited			cTnC	NULL		NH2-terminal domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_24_16681_s_63	10358006	4 Taken together, these results allow us to propose that both nonphosphorylated and phosphorylated forms of cTnI bind to the COOH-terminal domain of cTnC with the nonphosphorylated form making limited contacts with the NH2-terminal domain of cTnC.	bind
26336	1	8101	6	13	NULL	NULL	NULL	DNA polymerase	GP		is encoded by					SP01	Organism	Bacillus subtilis phage			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_39_24207_s_175	8798663	4 The DNA polymerase encoded by SP01, a  Bacillus subtilis phage, contains a domain of approximately 45 residues that resemble the putative thioredoxin binding domain of T7 DNA polymerase ( 42).	bind
26337	2	8101	6	13	NULL	NULL	NULL	DNA polymerase	GP		resemble			45 residue domain		T7 DNA polymerase	GP	putative	thioredoxin binding domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_39_24207_s_175	8798663	4 The DNA polymerase encoded by SP01, a  Bacillus subtilis phage, contains a domain of approximately 45 residues that resemble the putative thioredoxin binding domain of T7 DNA polymerase ( 42).	bind
32180	1	8101	7	NULL	NULL	0	NULL	SP01	NULL	Bacillus subtilis phage	encodes	NULL				DNA polymerase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_39_24207_s_175	8798663	4 The DNA polymerase encoded by SP01, a  Bacillus subtilis phage, contains a domain of approximately 45 residues that resemble the putative thioredoxin binding domain of T7 DNA polymerase ( 42).	bind
32181	2	8101	7	10	NULL	0	NULL	DNA polymerase			resemble			45 residues		T7 DNA polymerase		putative	thioredoxin binding domain of		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_39_24207_s_175	8798663	4 The DNA polymerase encoded by SP01, a  Bacillus subtilis phage, contains a domain of approximately 45 residues that resemble the putative thioredoxin binding domain of T7 DNA polymerase ( 42).	bind
26338	1	8102	6	13	NULL	NULL	NULL	nNOS	GP		bind					L-canavanine	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_36_25218_s_187	10464242	4 The modestly decreased binding affinity of nNOS for L-canavanine is attributed to loss of this H-bond.	bind
26339	2	8102	6	13	NULL	NULL	NULL			loss of	decreases		modestly	H-bond		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_36_25218_s_187	10464242	4 The modestly decreased binding affinity of nNOS for L-canavanine is attributed to loss of this H-bond.	bind
32182	1	8102	7	NULL	NULL	0	NULL	nNOS	NULL		bind	NULL				L-canavanine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_36_25218_s_187	10464242	4 The modestly decreased binding affinity of nNOS for L-canavanine is attributed to loss of this H-bond.	bind
32183	2	8102	7	NULL	NULL	0	NULL	statement 1	NULL	decreased affinity of	is attributed to	NULL				 H-bond	NULL	loss of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_36_25218_s_187	10464242	4 The modestly decreased binding affinity of nNOS for L-canavanine is attributed to loss of this H-bond.	bind
26781	1	8103	6	13	NULL	NULL	NULL	Ess1	GP		reconfigures							phosphorylated	CTD		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_44_31583_s_151	10531363	4 The possibility that Ess1 reconfigures the phosphorylated CTD though processive isomerization of its proline residues certainly adds an unexpected twist to the investigation of eukaryotic pre-mRNA transcription and 3''-end formation.	bind
26782	2	8103	6	13	NULL	NULL	NULL	statement 1	Process		occurs through							processive isomerization of	proline residues		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_44_31583_s_151	10531363	4 The possibility that Ess1 reconfigures the phosphorylated CTD though processive isomerization of its proline residues certainly adds an unexpected twist to the investigation of eukaryotic pre-mRNA transcription and 3''-end formation.	bind
32184	1	8103	7	NULL	NULL	0	NULL	Ess1	NULL		reconfigures 	NULL					NULL	phosphorylated	CTD		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_44_31583_s_151	10531363	4 The possibility that Ess1 reconfigures the phosphorylated CTD though processive isomerization of its proline residues certainly adds an unexpected twist to the investigation of eukaryotic pre-mRNA transcription and 3''-end formation.	bind
32185	2	8103	7	NULL	NULL	0	NULL	statement 1	NULL		occurs through	NULL					NULL	 processive isomerization of 	 proline residues 		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_44_31583_s_151	10531363	4 The possibility that Ess1 reconfigures the phosphorylated CTD though processive isomerization of its proline residues certainly adds an unexpected twist to the investigation of eukaryotic pre-mRNA transcription and 3''-end formation.	bind
26340	1	8104	6	13	NULL	NULL	NULL	MxA	GP		bind					RNP structure	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_7_4370_s_224	9933640	4 The present data strongly suggest that MxA binds to the RNP structure by recognizing its major protein component, NP.	bind
26341	2	8104	6	13	NULL	NULL	NULL	MxA	GP		recognize					protein component NP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_7_4370_s_224	9933640	4 The present data strongly suggest that MxA binds to the RNP structure by recognizing its major protein component, NP.	bind
26342	3	8104	6	13	NULL	NULL	NULL	statement 1	Process		occurs via					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_7_4370_s_224	9933640	4 The present data strongly suggest that MxA binds to the RNP structure by recognizing its major protein component, NP.	bind
32186	1	8104	7	NULL	NULL	0	NULL	MxA	NULL		binds to	NULL				RNP structure	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_7_4370_s_224	9933640	4 The present data strongly suggest that MxA binds to the RNP structure by recognizing its major protein component, NP.	bind
32187	2	8104	7	10	NULL	0	NULL	MxA	NULL		recognizes	NULL				protein component NP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_7_4370_s_224	9933640	4 The present data strongly suggest that MxA binds to the RNP structure by recognizing its major protein component, NP.	bind
46565	3	8104	7	10	NULL	0	NULL	statement 1	NULL		occurs via	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_7_4370_s_224	9933640	4 The present data strongly suggest that MxA binds to the RNP structure by recognizing its major protein component, NP.	bind
26343	1	8105	6	13	NULL	NULL	NULL	EKLF	GP		bind					LCR gene	GP			promoter	NULL	yolk sac	NULL	NULL	NULL	NULL	gw70_jbiolchem_281_23_16052_s_148	16606611	4 Therefore, EKLF binding to both LCR and globin gene promoter sequences in the yolk sac, fetal liver, and bone marrow appears to be critical for correct globin gene regulation during development.	bind
26344	2	8105	6	13	NULL	NULL	NULL	EKLF	GP		bind					LCR gene	GP			promoter	NULL	fetal liver	NULL	NULL	NULL	NULL	gw70_jbiolchem_281_23_16052_s_148	16606611	4 Therefore, EKLF binding to both LCR and globin gene promoter sequences in the yolk sac, fetal liver, and bone marrow appears to be critical for correct globin gene regulation during development.	bind
26345	3	8105	6	13	NULL	NULL	NULL	EKLF	GP		bind					LCR gene	GP			promoter	NULL	bone marrow	NULL	NULL	NULL	NULL	gw70_jbiolchem_281_23_16052_s_148	16606611	4 Therefore, EKLF binding to both LCR and globin gene promoter sequences in the yolk sac, fetal liver, and bone marrow appears to be critical for correct globin gene regulation during development.	bind
26346	4	8105	6	13	NULL	NULL	NULL	EKLF	GP		bind					globin gene	GP			promoter	NULL	yolk sac	NULL	NULL	NULL	NULL	gw70_jbiolchem_281_23_16052_s_148	16606611	4 Therefore, EKLF binding to both LCR and globin gene promoter sequences in the yolk sac, fetal liver, and bone marrow appears to be critical for correct globin gene regulation during development.	bind
26347	5	8105	6	13	NULL	NULL	NULL	EKLF	GP		bind					globin gene	GP			promoter	NULL	fetal liver	NULL	NULL	NULL	NULL	gw70_jbiolchem_281_23_16052_s_148	16606611	4 Therefore, EKLF binding to both LCR and globin gene promoter sequences in the yolk sac, fetal liver, and bone marrow appears to be critical for correct globin gene regulation during development.	bind
26348	6	8105	6	13	NULL	NULL	NULL	EKLF	GP		bind					globin gene	GP			promoter	NULL	bone marrow	NULL	NULL	NULL	NULL	gw70_jbiolchem_281_23_16052_s_148	16606611	4 Therefore, EKLF binding to both LCR and globin gene promoter sequences in the yolk sac, fetal liver, and bone marrow appears to be critical for correct globin gene regulation during development.	bind
32189	1	8105	7	NULL	NULL	0	NULL	EKLF	NULL		bind	NULL				LCR gene	NULL			promoter	NULL	yolk sac	NULL	NULL	NULL	NULL	gw70_jbiolchem_281_23_16052_s_148	16606611	4 Therefore, EKLF binding to both LCR and globin gene promoter sequences in the yolk sac, fetal liver, and bone marrow appears to be critical for correct globin gene regulation during development.	bind
32190	2	8105	7	NULL	NULL	0	NULL	EKLF	NULL		bind	NULL				globin gene	NULL			promoter	NULL	yolk sac	NULL	NULL	NULL	NULL	gw70_jbiolchem_281_23_16052_s_148	16606611	4 Therefore, EKLF binding to both LCR and globin gene promoter sequences in the yolk sac, fetal liver, and bone marrow appears to be critical for correct globin gene regulation during development.	bind
32191	3	8105	7	NULL	NULL	0	NULL	EKLF	NULL		bind	NULL				LCR gene	NULL			promoter	NULL	fetal liver	0	NULL	NULL	NULL	gw70_jbiolchem_281_23_16052_s_148	16606611	4 Therefore, EKLF binding to both LCR and globin gene promoter sequences in the yolk sac, fetal liver, and bone marrow appears to be critical for correct globin gene regulation during development.	bind
32192	4	8105	7	NULL	NULL	0	NULL	EKLF	NULL		bind	NULL				globin gene	NULL			promoter	NULL	fetal liver	0	NULL	NULL	NULL	gw70_jbiolchem_281_23_16052_s_148	16606611	4 Therefore, EKLF binding to both LCR and globin gene promoter sequences in the yolk sac, fetal liver, and bone marrow appears to be critical for correct globin gene regulation during development.	bind
32193	5	8105	7	NULL	NULL	0	NULL	EKLF	NULL		bind	NULL				LCR gene	NULL			promoter	NULL	 bone marrow	0	NULL	NULL	NULL	gw70_jbiolchem_281_23_16052_s_148	16606611	4 Therefore, EKLF binding to both LCR and globin gene promoter sequences in the yolk sac, fetal liver, and bone marrow appears to be critical for correct globin gene regulation during development.	bind
32194	6	8105	7	NULL	NULL	0	NULL	EKLF	NULL		bind	NULL				globin gene	NULL			promoter	NULL	bone marrow	NULL	NULL	NULL	NULL	gw70_jbiolchem_281_23_16052_s_148	16606611	4 Therefore, EKLF binding to both LCR and globin gene promoter sequences in the yolk sac, fetal liver, and bone marrow appears to be critical for correct globin gene regulation during development.	bind
32195	7	8105	7	NULL	NULL	0	NULL	statement 1	NULL		is critical for	NULL				globin gene	NULL	regulation of			NULL	during development	0	NULL	NULL	NULL	gw70_jbiolchem_281_23_16052_s_148	16606611	4 Therefore, EKLF binding to both LCR and globin gene promoter sequences in the yolk sac, fetal liver, and bone marrow appears to be critical for correct globin gene regulation during development.	bind
32196	8	8105	7	NULL	NULL	0	NULL	statement 2	NULL		is critical for	NULL				globin gene	NULL	regulation of			NULL	during development	0	NULL	NULL	NULL	gw70_jbiolchem_281_23_16052_s_148	16606611	4 Therefore, EKLF binding to both LCR and globin gene promoter sequences in the yolk sac, fetal liver, and bone marrow appears to be critical for correct globin gene regulation during development.	bind
32197	9	8105	7	NULL	NULL	0	NULL	statement 3	NULL		is critical for	NULL				globin gene	NULL	regulation of			NULL	during development	0	NULL	NULL	NULL	gw70_jbiolchem_281_23_16052_s_148	16606611	4 Therefore, EKLF binding to both LCR and globin gene promoter sequences in the yolk sac, fetal liver, and bone marrow appears to be critical for correct globin gene regulation during development.	bind
32198	10	8105	7	NULL	NULL	0	NULL	statement 4	NULL		is critical for	NULL				globin gene	NULL	regulation of			NULL	during development	0	NULL	NULL	NULL	gw70_jbiolchem_281_23_16052_s_148	16606611	4 Therefore, EKLF binding to both LCR and globin gene promoter sequences in the yolk sac, fetal liver, and bone marrow appears to be critical for correct globin gene regulation during development.	bind
32199	11	8105	7	NULL	NULL	0	NULL	statement 5	NULL		is critical for	NULL				globin gene	NULL	regulation of			NULL	during development	0	NULL	NULL	NULL	gw70_jbiolchem_281_23_16052_s_148	16606611	4 Therefore, EKLF binding to both LCR and globin gene promoter sequences in the yolk sac, fetal liver, and bone marrow appears to be critical for correct globin gene regulation during development.	bind
32200	12	8105	7	NULL	NULL	0	NULL	statement 6	NULL		is critical for	NULL				globin gene	NULL	regulation of			NULL	during development	0	NULL	NULL	NULL	gw70_jbiolchem_281_23_16052_s_148	16606611	4 Therefore, EKLF binding to both LCR and globin gene promoter sequences in the yolk sac, fetal liver, and bone marrow appears to be critical for correct globin gene regulation during development.	bind
26349	1	8106	6	13	NULL	NULL	NULL	synaptotagmin I	GP		bind					synaptotagmin I	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_49_32966_s_101	9830048	4 Therefore, the analysis of the C2B-effector recognition site, described below, is focused on the self-association of synaptotagmin I and the binding of synaptotagmin to AP-2.	bind
26350	2	8106	6	13	NULL	NULL	NULL	synaptotagmin	GP		bind					AP-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_49_32966_s_101	9830048	4 Therefore, the analysis of the C2B-effector recognition site, described below, is focused on the self-association of synaptotagmin I and the binding of synaptotagmin to AP-2.	bind
32270	1	8106	7	NULL	NULL	0	NULL	synaptotagmin I 	NULL		self-associate with	NULL				synaptotagmin I 	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_49_32966_s_101	9830048	4 Therefore, the analysis of the C2B-effector recognition site, described below, is focused on the self-association of synaptotagmin I and the binding of synaptotagmin to AP-2.	bind
32271	2	8106	7	NULL	NULL	0	NULL	synaptotagmin 	NULL		bind	NULL				AP-2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_49_32966_s_101	9830048	4 Therefore, the analysis of the C2B-effector recognition site, described below, is focused on the self-association of synaptotagmin I and the binding of synaptotagmin to AP-2.	bind
26353	1	8107	6	13	NULL	NULL	NULL	FX cluster	GP		is a prerequisite for					PsaC	GP	binding of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_23_20355_s_288	11914374	4 These  in vitro studies, therefore, show that the FX cluster is a prerequisite for the binding of PsaC, which, in turn, is required for the binding of PsaD and PsaE.	bind
26354	2	8107	6	13	NULL	NULL	NULL	PsaD	GP		bind					PsaE	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_23_20355_s_288	11914374	4 These  in vitro studies, therefore, show that the FX cluster is a prerequisite for the binding of PsaC, which, in turn, is required for the binding of PsaD and PsaE.	bind
26355	3	8107	6	13	NULL	NULL	NULL	statement 1	Process		is required for					statement 2	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_23_20355_s_288	11914374	4 These  in vitro studies, therefore, show that the FX cluster is a prerequisite for the binding of PsaC, which, in turn, is required for the binding of PsaD and PsaE.	bind
32272	1	8107	7	NULL	NULL	0	NULL	FX cluster	NULL		is a prerequisite for	NULL				PsaC	NULL	binding of			NULL	in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_277_23_20355_s_288	11914374	4 These  in vitro studies, therefore, show that the FX cluster is a prerequisite for the binding of PsaC, which, in turn, is required for the binding of PsaD and PsaE.	bind
32273	2	8107	7	NULL	NULL	0	NULL	PsaD	NULL		bind	NULL				PsaE	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_23_20355_s_288	11914374	4 These  in vitro studies, therefore, show that the FX cluster is a prerequisite for the binding of PsaC, which, in turn, is required for the binding of PsaD and PsaE.	bind
32274	3	8107	7	NULL	NULL	0	NULL	PsaC	NULL		is required for	NULL				statement 2	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_23_20355_s_288	11914374	4 These  in vitro studies, therefore, show that the FX cluster is a prerequisite for the binding of PsaC, which, in turn, is required for the binding of PsaD and PsaE.	bind
26783	1	8108	6	13	NULL	NULL	NULL	Spo0B	GP		bind					Spo0F	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_23_20483_s_267	11923303	4 These observations prompted us to predict that Spo0E and Rap phosphatases may assume a structural conformation with strong similarity to the helical organization of the Spo0B binding interface to Spo0F.	bind
32275	1	8108	7	NULL	NULL	0	NULL	Spo0B	NULL		bind	NULL				Spo0F	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_23_20483_s_267	11923303	4 These observations prompted us to predict that Spo0E and Rap phosphatases may assume a structural conformation with strong similarity to the helical organization of the Spo0B binding interface to Spo0F.	bind
26784	1	8109	6	13	NULL	NULL	NULL	mAChR	GP		dissociates from			M1 		TRPC6 channesls	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_32035_s_330	15994335	4 These observations, together with the results described above, imply that disassociation of M1 mAChRs from TRPC6 channels requires three sequential events as follows: 1) phosphorylation of TRPC6 channels on Ser768/714 by PKC; 2) binding of FKBP12 to a site immediately adjacent to Ser768/714; and 3) dephosphorylation of Ser768/714 by calcineurin targeted to the TRPC6/FKBP12 anchor.	bind
26785	2	8109	6	13	NULL	NULL	NULL	PKC	GP		phosphorylates					TRPC6	GP		Ser768/714		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_32035_s_330	15994335	4 These observations, together with the results described above, imply that disassociation of M1 mAChRs from TRPC6 channels requires three sequential events as follows: 1) phosphorylation of TRPC6 channels on Ser768/714 by PKC; 2) binding of FKBP12 to a site immediately adjacent to Ser768/714; and 3) dephosphorylation of Ser768/714 by calcineurin targeted to the TRPC6/FKBP12 anchor.	bind
26877	3	8109	6	13	NULL	NULL	NULL	FKB12	GP		bind					TRPC6	GP	site immediately adjacent to	Ser768/714		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_32035_s_330	15994335	4 These observations, together with the results described above, imply that disassociation of M1 mAChRs from TRPC6 channels requires three sequential events as follows: 1) phosphorylation of TRPC6 channels on Ser768/714 by PKC; 2) binding of FKBP12 to a site immediately adjacent to Ser768/714; and 3) dephosphorylation of Ser768/714 by calcineurin targeted to the TRPC6/FKBP12 anchor.	bind
26878	4	8109	6	13	NULL	NULL	NULL	calcineurin	GP		is targeted to					TRPC6/FKBP12 anchor	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_32035_s_330	15994335	4 These observations, together with the results described above, imply that disassociation of M1 mAChRs from TRPC6 channels requires three sequential events as follows: 1) phosphorylation of TRPC6 channels on Ser768/714 by PKC; 2) binding of FKBP12 to a site immediately adjacent to Ser768/714; and 3) dephosphorylation of Ser768/714 by calcineurin targeted to the TRPC6/FKBP12 anchor.	bind
26879	5	8109	6	13	NULL	NULL	NULL	statement 4	Process		dephosphorylates					TRPC6	GP		Ser768/714		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_32035_s_330	15994335	4 These observations, together with the results described above, imply that disassociation of M1 mAChRs from TRPC6 channels requires three sequential events as follows: 1) phosphorylation of TRPC6 channels on Ser768/714 by PKC; 2) binding of FKBP12 to a site immediately adjacent to Ser768/714; and 3) dephosphorylation of Ser768/714 by calcineurin targeted to the TRPC6/FKBP12 anchor.	bind
26880	6	8109	6	13	NULL	NULL	NULL	statement 1	Process		occurs via					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_32035_s_330	15994335	4 These observations, together with the results described above, imply that disassociation of M1 mAChRs from TRPC6 channels requires three sequential events as follows: 1) phosphorylation of TRPC6 channels on Ser768/714 by PKC; 2) binding of FKBP12 to a site immediately adjacent to Ser768/714; and 3) dephosphorylation of Ser768/714 by calcineurin targeted to the TRPC6/FKBP12 anchor.	bind
26881	7	8109	6	13	NULL	NULL	NULL	statement 1	Process		occurs via					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_32035_s_330	15994335	4 These observations, together with the results described above, imply that disassociation of M1 mAChRs from TRPC6 channels requires three sequential events as follows: 1) phosphorylation of TRPC6 channels on Ser768/714 by PKC; 2) binding of FKBP12 to a site immediately adjacent to Ser768/714; and 3) dephosphorylation of Ser768/714 by calcineurin targeted to the TRPC6/FKBP12 anchor.	bind
26882	8	8109	6	13	NULL	NULL	NULL	statement 1	Process		occurs via					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_32035_s_330	15994335	4 These observations, together with the results described above, imply that disassociation of M1 mAChRs from TRPC6 channels requires three sequential events as follows: 1) phosphorylation of TRPC6 channels on Ser768/714 by PKC; 2) binding of FKBP12 to a site immediately adjacent to Ser768/714; and 3) dephosphorylation of Ser768/714 by calcineurin targeted to the TRPC6/FKBP12 anchor.	bind
32280	1	8109	7	NULL	NULL	0	NULL	PKC	NULL		phosphorylates	NULL				TRPC6 channels	NULL		Ser768/714		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_36_32035_s_330	15994335	4 These observations, together with the results described above, imply that disassociation of M1 mAChRs from TRPC6 channels requires three sequential events as follows: 1) phosphorylation of TRPC6 channels on Ser768/714 by PKC; 2) binding of FKBP12 to a site immediately adjacent to Ser768/714; and 3) dephosphorylation of Ser768/714 by calcineurin targeted to the TRPC6/FKBP12 anchor.	bind
32281	2	8109	7	10	NULL	0	NULL	FKBP12 	NULL		bind	NULL				TRPC6	NULL	site adjacent to	 Ser768/714		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_32035_s_330	15994335	4 These observations, together with the results described above, imply that disassociation of M1 mAChRs from TRPC6 channels requires three sequential events as follows: 1) phosphorylation of TRPC6 channels on Ser768/714 by PKC; 2) binding of FKBP12 to a site immediately adjacent to Ser768/714; and 3) dephosphorylation of Ser768/714 by calcineurin targeted to the TRPC6/FKBP12 anchor.	bind
32282	3	8109	7	NULL	NULL	0	NULL	calcineurin 	NULL		dephosphorylates	NULL					NULL		Ser768/714		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_36_32035_s_330	15994335	4 These observations, together with the results described above, imply that disassociation of M1 mAChRs from TRPC6 channels requires three sequential events as follows: 1) phosphorylation of TRPC6 channels on Ser768/714 by PKC; 2) binding of FKBP12 to a site immediately adjacent to Ser768/714; and 3) dephosphorylation of Ser768/714 by calcineurin targeted to the TRPC6/FKBP12 anchor.	bind
32283	4	8109	7	NULL	NULL	0	NULL	statement 3	NULL		is targeted to	NULL				TRPC6/FKBP12 anchor	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_36_32035_s_330	15994335	4 These observations, together with the results described above, imply that disassociation of M1 mAChRs from TRPC6 channels requires three sequential events as follows: 1) phosphorylation of TRPC6 channels on Ser768/714 by PKC; 2) binding of FKBP12 to a site immediately adjacent to Ser768/714; and 3) dephosphorylation of Ser768/714 by calcineurin targeted to the TRPC6/FKBP12 anchor.	bind
32284	5	8109	7	NULL	NULL	0	NULL	M1 mAChRs	NULL		dissociates from	NULL				 TRPC6 channels 	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_36_32035_s_330	15994335	4 These observations, together with the results described above, imply that disassociation of M1 mAChRs from TRPC6 channels requires three sequential events as follows: 1) phosphorylation of TRPC6 channels on Ser768/714 by PKC; 2) binding of FKBP12 to a site immediately adjacent to Ser768/714; and 3) dephosphorylation of Ser768/714 by calcineurin targeted to the TRPC6/FKBP12 anchor.	bind
32285	6	8109	7	NULL	NULL	0	NULL	statement 5	NULL		requires	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_36_32035_s_330	15994335	4 These observations, together with the results described above, imply that disassociation of M1 mAChRs from TRPC6 channels requires three sequential events as follows: 1) phosphorylation of TRPC6 channels on Ser768/714 by PKC; 2) binding of FKBP12 to a site immediately adjacent to Ser768/714; and 3) dephosphorylation of Ser768/714 by calcineurin targeted to the TRPC6/FKBP12 anchor.	bind
32286	7	8109	7	NULL	NULL	0	NULL	statement 5	NULL		requires	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_36_32035_s_330	15994335	4 These observations, together with the results described above, imply that disassociation of M1 mAChRs from TRPC6 channels requires three sequential events as follows: 1) phosphorylation of TRPC6 channels on Ser768/714 by PKC; 2) binding of FKBP12 to a site immediately adjacent to Ser768/714; and 3) dephosphorylation of Ser768/714 by calcineurin targeted to the TRPC6/FKBP12 anchor.	bind
32287	8	8109	7	NULL	NULL	0	NULL	statement 5	NULL		requires	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_36_32035_s_330	15994335	4 These observations, together with the results described above, imply that disassociation of M1 mAChRs from TRPC6 channels requires three sequential events as follows: 1) phosphorylation of TRPC6 channels on Ser768/714 by PKC; 2) binding of FKBP12 to a site immediately adjacent to Ser768/714; and 3) dephosphorylation of Ser768/714 by calcineurin targeted to the TRPC6/FKBP12 anchor.	bind
26357	1	8110	6	13	NULL	NULL	NULL	VLA-4	GP		bind					VCAM-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_51_51203_s_140	14532283	4 These results were surprising in light of the fact that VLA-4 binds this mAb at an affinity orders of magnitude higherR than it binds VCAM-1 ( ).	bind
32289	1	8110	7	10	NULL	0	NULL	VLA-4	NULL		binds	NULL				VCAM-1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_51_51203_s_140	14532283	4 These results were surprising in light of the fact that VLA-4 binds this mAb at an affinity orders of magnitude higherR than it binds VCAM-1 ( ).	bind
26359	1	8111	6	13	NULL	NULL	NULL	DnaA protein	GP	B. subtilis	does not bind					DnaB	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34255_s_220	9852089	4 This interpretation is supported by the observation that  B. subtilis DnaA protein failed to bind to DnaB.	bind
32291	1	8111	7	NULL	NULL	0	NULL	DnaA protein	NULL	 B. subtilis	does not bind	NULL				DnaB	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_51_34255_s_220	9852089	4 This interpretation is supported by the observation that  B. subtilis DnaA protein failed to bind to DnaB.	bind
55832	1	8112	6	13	NULL	NULL	NULL	P25 peptide	GP		bind					uPAR	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_14_9450_s_329	16461772	4 This is not particularly surprising, because the P25 peptide binds uPAR in a site distinct from both the vitronectin and uPA binding sites ( ).	bind
32292	1	8112	7	NULL	NULL	0	NULL	P25 peptide	NULL		binds	NULL				uPAR	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_14_9450_s_329	16461772	4 This is not particularly surprising, because the P25 peptide binds uPAR in a site distinct from both the vitronectin and uPA binding sites ( ).	bind
32293	2	8112	7	NULL	NULL	0	NULL	P25 peptide	NULL	binding site of	is distinct from	NULL				uPAR	NULL		uPA binding site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_14_9450_s_329	16461772	4 This is not particularly surprising, because the P25 peptide binds uPAR in a site distinct from both the vitronectin and uPA binding sites ( ).	bind
32294	3	8112	7	NULL	NULL	0	NULL	P25 peptide	NULL	binding site of	is distinct from	NULL				uPAR	NULL		vitronectin binding site		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_14_9450_s_329	16461772	4 This is not particularly surprising, because the P25 peptide binds uPAR in a site distinct from both the vitronectin and uPA binding sites ( ).	bind
26364	1	8113	6	13	NULL	NULL	NULL	TGF-beta1	GP		bind					TbetaR-II	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_17_11506_s_250	16492675	4 This suggests that the formation of Complex I (with a high ratio of TGF-beta1 binding to TbetaR-II and TbetaR-I) is a default process and that the formation of Complex II ( e.g. induced by heparan sulfate) is a regulatory event.	bind
26883	2	8113	6	13	NULL	NULL	NULL	TGF-beta1	GP		bind					TbetaR-I	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_17_11506_s_250	16492675	4 This suggests that the formation of Complex I (with a high ratio of TGF-beta1 binding to TbetaR-II and TbetaR-I) is a default process and that the formation of Complex II ( e.g. induced by heparan sulfate) is a regulatory event.	bind
26884	3	8113	6	13	NULL	NULL	NULL	Complex I	GP		consists of					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_17_11506_s_250	16492675	4 This suggests that the formation of Complex I (with a high ratio of TGF-beta1 binding to TbetaR-II and TbetaR-I) is a default process and that the formation of Complex II ( e.g. induced by heparan sulfate) is a regulatory event.	bind
26885	4	8113	6	13	NULL	NULL	NULL	Complex I	GP		consists of					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_17_11506_s_250	16492675	4 This suggests that the formation of Complex I (with a high ratio of TGF-beta1 binding to TbetaR-II and TbetaR-I) is a default process and that the formation of Complex II ( e.g. induced by heparan sulfate) is a regulatory event.	bind
26886	5	8113	6	13	NULL	NULL	NULL	complex II	GP	formation of	is induced by					heparan sulfate	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_17_11506_s_250	16492675	4 This suggests that the formation of Complex I (with a high ratio of TGF-beta1 binding to TbetaR-II and TbetaR-I) is a default process and that the formation of Complex II ( e.g. induced by heparan sulfate) is a regulatory event.	bind
32295	1	8113	7	NULL	NULL	0	NULL	TGF-beta1 	NULL		bind	NULL				TbetaR-II	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_17_11506_s_250	16492675	4 This suggests that the formation of Complex I (with a high ratio of TGF-beta1 binding to TbetaR-II and TbetaR-I) is a default process and that the formation of Complex II ( e.g. induced by heparan sulfate) is a regulatory event.	bind
32296	2	8113	7	NULL	NULL	0	NULL	TGF-beta1	NULL		bind	NULL				 TbetaR-I	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_17_11506_s_250	16492675	4 This suggests that the formation of Complex I (with a high ratio of TGF-beta1 binding to TbetaR-II and TbetaR-I) is a default process and that the formation of Complex II ( e.g. induced by heparan sulfate) is a regulatory event.	bind
32297	3	8113	7	NULL	NULL	0	NULL	Complex I	NULL		consist of	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_17_11506_s_250	16492675	4 This suggests that the formation of Complex I (with a high ratio of TGF-beta1 binding to TbetaR-II and TbetaR-I) is a default process and that the formation of Complex II ( e.g. induced by heparan sulfate) is a regulatory event.	bind
32298	4	8113	7	NULL	NULL	0	NULL	Complex I	NULL		consist of	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_17_11506_s_250	16492675	4 This suggests that the formation of Complex I (with a high ratio of TGF-beta1 binding to TbetaR-II and TbetaR-I) is a default process and that the formation of Complex II ( e.g. induced by heparan sulfate) is a regulatory event.	bind
32300	5	8113	7	10	NULL	0	NULL	heparan sulfate	NULL		induce	NULL				Complex II	NULL	formation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_17_11506_s_250	16492675	4 This suggests that the formation of Complex I (with a high ratio of TGF-beta1 binding to TbetaR-II and TbetaR-I) is a default process and that the formation of Complex II ( e.g. induced by heparan sulfate) is a regulatory event.	bind
26365	1	8114	6	13	NULL	NULL	NULL	Stm1p	GP		bind					Pu triplexes	NucleicAcid				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_8_5573_s_286	10681538	4 This would suggest that Stm1p could bind Pu triplexes  in vivo, should they occur.	bind
32301	1	8114	7	NULL	NULL	0	NULL	Stm1p	NULL		bind	NULL				Pu triplexes	NULL				NULL	in vivo	0	NULL	NULL	NULL	gw60_jbiolchem_275_8_5573_s_286	10681538	4 This would suggest that Stm1p could bind Pu triplexes  in vivo, should they occur.	bind
26887	1	8115	6	13	NULL	NULL	NULL	FAK	GP		bind			vinculin homologous sequences		paxillin	GP		FAK binding site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_51_36684_s_333	10593973	4 Thus one can imagine that vinculin homologous sequences in FAK bind to the first FAK-binding site in paxillin and a second, unrelated sequence in FAK binds to the second paxillin interaction site.	bind
26888	2	8115	6	13	NULL	NULL	NULL	FAK	GP	unrelated sequence	bind								paxillin interaction site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_51_36684_s_333	10593973	4 Thus one can imagine that vinculin homologous sequences in FAK bind to the first FAK-binding site in paxillin and a second, unrelated sequence in FAK binds to the second paxillin interaction site.	bind
32302	1	8115	7	10	NULL	0	NULL	FAK	NULL		bind	NULL		vinculin homologous sequence		paxillin	NULL		FAK-binding site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_51_36684_s_333	10593973	4 Thus one can imagine that vinculin homologous sequences in FAK bind to the first FAK-binding site in paxillin and a second, unrelated sequence in FAK binds to the second paxillin interaction site.	bind
32304	3	8115	7	10	NULL	0	NULL	FAK	NULL	unrelated sequence	bind	NULL				paxillin	NULL		second interaction site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_51_36684_s_333	10593973	4 Thus one can imagine that vinculin homologous sequences in FAK bind to the first FAK-binding site in paxillin and a second, unrelated sequence in FAK binds to the second paxillin interaction site.	bind
26384	1	8116	6	13	NULL	NULL	NULL	DP1	GP	DN binding form of 	bind					E2F	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_27_19011_s_152	10383401	4 To test our hypothesis, we expressed a DN binding form of DP1, an obligate binding partner to E2F, wild type, and deletion mutants of DP1, which do not display DN characteristics ( 23).	bind
32305	1	8116	7	NULL	NULL	0	NULL	DP1	NULL	DN binding form	binds	NULL				E2F	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_27_19011_s_152	10383401	4 To test our hypothesis, we expressed a DN binding form of DP1, an obligate binding partner to E2F, wild type, and deletion mutants of DP1, which do not display DN characteristics ( 23).	bind
26385	1	8117	6	13	NULL	NULL	NULL	Runx2	GP		bind					C/EBPbeta	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_32_22695_s_345	16772287	4 Together these results indicate that binding of Runx2 and C/EBPbeta is one of the early events during chromatin remodeling and transcriptional activation of the OC gene.	bind
26386	2	8117	6	13	NULL	NULL	NULL	statement 1	Process		occurs during					chromatin remodeling	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_32_22695_s_345	16772287	4 Together these results indicate that binding of Runx2 and C/EBPbeta is one of the early events during chromatin remodeling and transcriptional activation of the OC gene.	bind
26392	3	8117	6	13	NULL	NULL	NULL	statement 1	Process		occurs during					OC gene	GP	transcriptional activation of 			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_32_22695_s_345	16772287	4 Together these results indicate that binding of Runx2 and C/EBPbeta is one of the early events during chromatin remodeling and transcriptional activation of the OC gene.	bind
32308	1	8117	7	NULL	NULL	0	NULL	Runx2	NULL		binds	NULL				C/EBPbeta	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_22695_s_345	16772287	4 Together these results indicate that binding of Runx2 and C/EBPbeta is one of the early events during chromatin remodeling and transcriptional activation of the OC gene.	bind
32309	2	8117	7	NULL	NULL	0	NULL	statement 1	NULL		occurs during	NULL				chromatin remodeling	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_22695_s_345	16772287	4 Together these results indicate that binding of Runx2 and C/EBPbeta is one of the early events during chromatin remodeling and transcriptional activation of the OC gene.	bind
32310	3	8117	7	NULL	NULL	0	NULL	statement 1	NULL		occurs during	NULL				OC gene	NULL	transcriptional activation of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_22695_s_345	16772287	4 Together these results indicate that binding of Runx2 and C/EBPbeta is one of the early events during chromatin remodeling and transcriptional activation of the OC gene.	bind
26393	1	8118	6	13	NULL	NULL	NULL	Cx43	GP		dissociates from					ZO-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_2_215_s_182	14699011	4 Toyofuku et al 4 argued that dissociation of Cx43 from ZO-1 was secondary to tyrosine phosphorylation of Cx43CT by binding of the SH2 domain of c-Src.	bind
26394	2	8118	6	13	NULL	NULL	NULL	c-Src	GP		bind			SH2 domain		Cx43CT	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_2_215_s_182	14699011	4 Toyofuku et al 4 argued that dissociation of Cx43 from ZO-1 was secondary to tyrosine phosphorylation of Cx43CT by binding of the SH2 domain of c-Src.	bind
55833	3	8118	6	13	NULL	NULL	NULL	statement 2	Process		phosphorylates					Cx43CT	GP		tyrosine		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_2_215_s_182	14699011	4 Toyofuku et al 4 argued that dissociation of Cx43 from ZO-1 was secondary to tyrosine phosphorylation of Cx43CT by binding of the SH2 domain of c-Src.	bind
55834	4	8118	6	13	NULL	NULL	NULL	statement 1	Process		is secondary to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_2_215_s_182	14699011	4 Toyofuku et al 4 argued that dissociation of Cx43 from ZO-1 was secondary to tyrosine phosphorylation of Cx43CT by binding of the SH2 domain of c-Src.	bind
32311	1	8118	7	NULL	NULL	0	NULL	Cx43	NULL		dissociates from	NULL				 ZO-1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_2_215_s_182	14699011	4 Toyofuku et al 4 argued that dissociation of Cx43 from ZO-1 was secondary to tyrosine phosphorylation of Cx43CT by binding of the SH2 domain of c-Src.	bind
32312	2	8118	7	NULL	NULL	0	NULL	c-Src	NULL		bind	NULL		SH2 domain		Cx43CT	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_2_215_s_182	14699011	4 Toyofuku et al 4 argued that dissociation of Cx43 from ZO-1 was secondary to tyrosine phosphorylation of Cx43CT by binding of the SH2 domain of c-Src.	bind
32313	3	8118	7	NULL	NULL	0	NULL	statement 2	NULL		phosphorylates	NULL				Cx43CT	NULL		tyrosine		NULL		0	NULL	NULL	NULL	gw70_circulationres_94_2_215_s_182	14699011	4 Toyofuku et al 4 argued that dissociation of Cx43 from ZO-1 was secondary to tyrosine phosphorylation of Cx43CT by binding of the SH2 domain of c-Src.	bind
32314	4	8118	7	NULL	NULL	0	NULL	statement 1	NULL		is secondary to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_2_215_s_182	14699011	4 Toyofuku et al 4 argued that dissociation of Cx43 from ZO-1 was secondary to tyrosine phosphorylation of Cx43CT by binding of the SH2 domain of c-Src.	bind
26395	1	8119	6	13	NULL	NULL	NULL	transmembrane protein	GP		bind					factor VIIa	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_12_1217_s_17	15976319	4 Upon exposure to blood, the transmembrane protein binds and allosterically activates factor VIIa (FVIIa).	bind
26396	2	8119	6	13	NULL	NULL	NULL	transmembrane protein	GP		activates		allosterically			factor VIIa	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_12_1217_s_17	15976319	4 Upon exposure to blood, the transmembrane protein binds and allosterically activates factor VIIa (FVIIa).	bind
26397	3	8119	6	13	NULL	NULL	NULL	FVIIa	GP		is					factor VIIa	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_12_1217_s_17	15976319	4 Upon exposure to blood, the transmembrane protein binds and allosterically activates factor VIIa (FVIIa).	bind
26398	4	8119	6	13	NULL	NULL	NULL	statement 1	Process		occurs upon exposure to					blood	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_12_1217_s_17	15976319	4 Upon exposure to blood, the transmembrane protein binds and allosterically activates factor VIIa (FVIIa).	bind
26399	5	8119	6	13	NULL	NULL	NULL	statement 2	Process		occurs upon exposure to					blood	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_12_1217_s_17	15976319	4 Upon exposure to blood, the transmembrane protein binds and allosterically activates factor VIIa (FVIIa).	bind
32315	1	8119	7	NULL	NULL	0	NULL	transmembrane protein	NULL		bind	NULL				FVIIa	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_12_1217_s_17	15976319	4 Upon exposure to blood, the transmembrane protein binds and allosterically activates factor VIIa (FVIIa).	bind
32316	2	8119	7	NULL	NULL	0	NULL	statement 1	NULL		activates	NULL	allosterically			FVIIa	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_12_1217_s_17	15976319	4 Upon exposure to blood, the transmembrane protein binds and allosterically activates factor VIIa (FVIIa).	bind
32317	3	8119	7	NULL	NULL	0	NULL	statement 1	NULL		occurs upon	NULL				blood	NULL	exposure to			NULL		0	NULL	NULL	NULL	gw70_circulationres_96_12_1217_s_17	15976319	4 Upon exposure to blood, the transmembrane protein binds and allosterically activates factor VIIa (FVIIa).	bind
32318	4	8119	7	NULL	NULL	0	NULL	statement 2	NULL		occurs upon	NULL				blood	NULL	exposure to			NULL		0	NULL	NULL	NULL	gw70_circulationres_96_12_1217_s_17	15976319	4 Upon exposure to blood, the transmembrane protein binds and allosterically activates factor VIIa (FVIIa).	bind
32319	5	8119	7	NULL	NULL	0	NULL	FVIIa	NULL		is	NULL				factor VIIa	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_12_1217_s_17	15976319	4 Upon exposure to blood, the transmembrane protein binds and allosterically activates factor VIIa (FVIIa).	bind
26400	1	8120	6	13	NULL	NULL	NULL	Vps9p	GP		bind					ubiquitin	GP	free			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_19826_s_274	12654912	4 Vps9p  binding to free ubiquitin has been demonstrated here; however, CUE domain  binding may be preferential toward protein-conjugated ubiquityl moieties and  thereby target Vps9p to ubiquitylated membrane proteins during endocytosis.	bind
26401	2	8120	6	13	NULL	NULL	NULL	Vps9p	GP		is targeted to					membrane proteins	GP	ubiquitylated			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_19826_s_274	12654912	4 Vps9p  binding to free ubiquitin has been demonstrated here; however, CUE domain  binding may be preferential toward protein-conjugated ubiquityl moieties and  thereby target Vps9p to ubiquitylated membrane proteins during endocytosis.	bind
26402	3	8120	6	13	NULL	NULL	NULL	statement 2	Process		occurs during					endocytosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_19826_s_274	12654912	4 Vps9p  binding to free ubiquitin has been demonstrated here; however, CUE domain  binding may be preferential toward protein-conjugated ubiquityl moieties and  thereby target Vps9p to ubiquitylated membrane proteins during endocytosis.	bind
32320	1	8120	7	NULL	NULL	0	NULL	 Vps9p	NULL		binds	NULL				Ubiquitin	NULL	free			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_22_19826_s_274	12654912	4 Vps9p  binding to free ubiquitin has been demonstrated here; however, CUE domain  binding may be preferential toward protein-conjugated ubiquityl moieties and  thereby target Vps9p to ubiquitylated membrane proteins during endocytosis.	bind
32321	2	8120	7	NULL	NULL	0	NULL		NULL		be preferred for	NULL	may	CUE domain		protein-conjugated ubiquityl moieties	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_22_19826_s_274	12654912	4 Vps9p  binding to free ubiquitin has been demonstrated here; however, CUE domain  binding may be preferential toward protein-conjugated ubiquityl moieties and  thereby target Vps9p to ubiquitylated membrane proteins during endocytosis.	bind
32322	3	8120	7	10	NULL	0	NULL	Vps9p			targeted to					membrane proteins		ubiquitylated 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_19826_s_274	12654912	4 Vps9p  binding to free ubiquitin has been demonstrated here; however, CUE domain  binding may be preferential toward protein-conjugated ubiquityl moieties and  thereby target Vps9p to ubiquitylated membrane proteins during endocytosis.	bind
32323	4	8120	7	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_22_19826_s_274	12654912	4 Vps9p  binding to free ubiquitin has been demonstrated here; however, CUE domain  binding may be preferential toward protein-conjugated ubiquityl moieties and  thereby target Vps9p to ubiquitylated membrane proteins during endocytosis.	bind
46566	5	8120	7	10	NULL	0	NULL	statement 3	NULL		occurs during	NULL				endocytosis	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_22_19826_s_274	12654912	4 Vps9p  binding to free ubiquitin has been demonstrated here; however, CUE domain  binding may be preferential toward protein-conjugated ubiquityl moieties and  thereby target Vps9p to ubiquitylated membrane proteins during endocytosis.	bind
26403	1	8121	6	13	NULL	NULL	NULL	substrates	GP	linear	contain							mutant		lox site	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_33_31092_s_277	11406627	4 We found that Cre efficiently binds, cleaves, and recombines linear substrates containing the same mutant  lox site as chi4 (L. Lee and P. D. Sadowski, unpublished data).	bind
26404	2	8121	6	13	NULL	NULL	NULL	Cre	GP		bind		efficiently			statement 1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_33_31092_s_277	11406627	4 We found that Cre efficiently binds, cleaves, and recombines linear substrates containing the same mutant  lox site as chi4 (L. Lee and P. D. Sadowski, unpublished data).	bind
26405	3	8121	6	13	NULL	NULL	NULL	Cre	GP		cleaves					statement 1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_33_31092_s_277	11406627	4 We found that Cre efficiently binds, cleaves, and recombines linear substrates containing the same mutant  lox site as chi4 (L. Lee and P. D. Sadowski, unpublished data).	bind
26406	4	8121	6	13	NULL	NULL	NULL	Cre	GP		recombines					statement 1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_33_31092_s_277	11406627	4 We found that Cre efficiently binds, cleaves, and recombines linear substrates containing the same mutant  lox site as chi4 (L. Lee and P. D. Sadowski, unpublished data).	bind
32348	1	8121	7	NULL	NULL	0	NULL	 Cre	NULL		binds	NULL	efficiently			linear substrate	NULL	mutant	lox site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_33_31092_s_277	11406627	4 We found that Cre efficiently binds, cleaves, and recombines linear substrates containing the same mutant  lox site as chi4 (L. Lee and P. D. Sadowski, unpublished data).	bind
32349	2	8121	7	NULL	NULL	0	NULL	Cre	NULL		cleaves	NULL	efficiently			linear substrate	NULL	mutant	lox site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_33_31092_s_277	11406627	4 We found that Cre efficiently binds, cleaves, and recombines linear substrates containing the same mutant  lox site as chi4 (L. Lee and P. D. Sadowski, unpublished data).	bind
32350	3	8121	7	NULL	NULL	0	NULL	Cre	NULL		recombines	NULL	efficiently			linear substrate	NULL	mutant	lox site		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_33_31092_s_277	11406627	4 We found that Cre efficiently binds, cleaves, and recombines linear substrates containing the same mutant  lox site as chi4 (L. Lee and P. D. Sadowski, unpublished data).	bind
32351	4	8121	7	NULL	NULL	0	NULL	Cre	NULL		binds	NULL	efficiently			chi4	NULL	mutant	lox site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_33_31092_s_277	11406627	4 We found that Cre efficiently binds, cleaves, and recombines linear substrates containing the same mutant  lox site as chi4 (L. Lee and P. D. Sadowski, unpublished data).	bind
32352	5	8121	7	NULL	NULL	0	NULL	Cre	NULL		cleaves	NULL	efficiently			chi4	NULL	mutant	lox site		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_33_31092_s_277	11406627	4 We found that Cre efficiently binds, cleaves, and recombines linear substrates containing the same mutant  lox site as chi4 (L. Lee and P. D. Sadowski, unpublished data).	bind
32353	6	8121	7	NULL	NULL	0	NULL	Cre	NULL		recombines	NULL	efficiently			chi4	NULL	mutant	lox site		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_33_31092_s_277	11406627	4 We found that Cre efficiently binds, cleaves, and recombines linear substrates containing the same mutant  lox site as chi4 (L. Lee and P. D. Sadowski, unpublished data).	bind
26889	1	8122	6	13	NULL	NULL	NULL	hypoxia/reoxygenation	Process		decreases					HSP60	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_21_2727_s_27	12438300	4 We hypothesized that HSP60 would decrease with hypoxia/reoxygenation, based on previous observations, 5 and that this would precipitate translocation of bax to the mitochondria and release of cytochrome c, based on our prior work showing that cytosolic HSP60 binds bax and that reduction in HSP60 precipitates apoptosis.	bind
26890	2	8122	6	13	NULL	NULL	NULL	bax	GP		translocate into					mitochondria	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_21_2727_s_27	12438300	4 We hypothesized that HSP60 would decrease with hypoxia/reoxygenation, based on previous observations, 5 and that this would precipitate translocation of bax to the mitochondria and release of cytochrome c, based on our prior work showing that cytosolic HSP60 binds bax and that reduction in HSP60 precipitates apoptosis.	bind
26891	3	8122	6	13	NULL	NULL	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_21_2727_s_27	12438300	4 We hypothesized that HSP60 would decrease with hypoxia/reoxygenation, based on previous observations, 5 and that this would precipitate translocation of bax to the mitochondria and release of cytochrome c, based on our prior work showing that cytosolic HSP60 binds bax and that reduction in HSP60 precipitates apoptosis.	bind
26892	4	8122	6	13	NULL	NULL	NULL	statement 1	Process		leads to					cytochrome c	GP	release of 			NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_21_2727_s_27	12438300	4 We hypothesized that HSP60 would decrease with hypoxia/reoxygenation, based on previous observations, 5 and that this would precipitate translocation of bax to the mitochondria and release of cytochrome c, based on our prior work showing that cytosolic HSP60 binds bax and that reduction in HSP60 precipitates apoptosis.	bind
26893	5	8122	6	13	NULL	NULL	NULL	HSP60	GP	cytosolic	bind					bax	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_21_2727_s_27	12438300	4 We hypothesized that HSP60 would decrease with hypoxia/reoxygenation, based on previous observations, 5 and that this would precipitate translocation of bax to the mitochondria and release of cytochrome c, based on our prior work showing that cytosolic HSP60 binds bax and that reduction in HSP60 precipitates apoptosis.	bind
26894	6	8122	6	13	NULL	NULL	NULL	HSP60	GP	reduction in	precipitates					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_21_2727_s_27	12438300	4 We hypothesized that HSP60 would decrease with hypoxia/reoxygenation, based on previous observations, 5 and that this would precipitate translocation of bax to the mitochondria and release of cytochrome c, based on our prior work showing that cytosolic HSP60 binds bax and that reduction in HSP60 precipitates apoptosis.	bind
32354	1	8122	7	NULL	NULL	0	NULL	HSP60 	NULL		decrease with	NULL				hypoxia/reoxygenation	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_21_2727_s_27	12438300	4 We hypothesized that HSP60 would decrease with hypoxia/reoxygenation, based on previous observations, 5 and that this would precipitate translocation of bax to the mitochondria and release of cytochrome c, based on our prior work showing that cytosolic HSP60 binds bax and that reduction in HSP60 precipitates apoptosis.	bind
32355	2	8122	7	10	NULL	0	NULL	bax			is translocated to					mitochondria					NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_21_2727_s_27	12438300	4 We hypothesized that HSP60 would decrease with hypoxia/reoxygenation, based on previous observations, 5 and that this would precipitate translocation of bax to the mitochondria and release of cytochrome c, based on our prior work showing that cytosolic HSP60 binds bax and that reduction in HSP60 precipitates apoptosis.	bind
32359	3	8122	7	NULL	NULL	0	NULL	statement 1	NULL		release	NULL				cytochrome c	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_21_2727_s_27	12438300	4 We hypothesized that HSP60 would decrease with hypoxia/reoxygenation, based on previous observations, 5 and that this would precipitate translocation of bax to the mitochondria and release of cytochrome c, based on our prior work showing that cytosolic HSP60 binds bax and that reduction in HSP60 precipitates apoptosis.	bind
32360	4	8122	7	NULL	NULL	0	NULL	HSP60	NULL	cytosolic	binds	NULL				bax	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_21_2727_s_27	12438300	4 We hypothesized that HSP60 would decrease with hypoxia/reoxygenation, based on previous observations, 5 and that this would precipitate translocation of bax to the mitochondria and release of cytochrome c, based on our prior work showing that cytosolic HSP60 binds bax and that reduction in HSP60 precipitates apoptosis.	bind
32361	5	8122	7	NULL	NULL	0	NULL	HSP60	NULL	reduction in	precipitates	NULL				apoptosis	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_21_2727_s_27	12438300	4 We hypothesized that HSP60 would decrease with hypoxia/reoxygenation, based on previous observations, 5 and that this would precipitate translocation of bax to the mitochondria and release of cytochrome c, based on our prior work showing that cytosolic HSP60 binds bax and that reduction in HSP60 precipitates apoptosis.	bind
55835	6	8122	7	10	NULL	0	NULL	statement 1			leads to					statement 2					NULL		0	NULL	NULL	NULL	gw60_circulation_106_21_2727_s_27	12438300	4 We hypothesized that HSP60 would decrease with hypoxia/reoxygenation, based on previous observations, 5 and that this would precipitate translocation of bax to the mitochondria and release of cytochrome c, based on our prior work showing that cytosolic HSP60 binds bax and that reduction in HSP60 precipitates apoptosis.	bind
26895	1	8124	6	13	NULL	NULL	NULL	4'F-DMA	Chemical		has affinity for					ERalpha	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_chem-res-toxicol_19_6_16780356_s_8	16780356	4'F-DMA shows ligand binding affinity to  estrogen receptor (ER)alpha and ERbeta with similarity to both raloxifene  and to DMA.	bind
26896	2	8124	6	13	NULL	NULL	NULL	ER	GP		is					estrogen receptor	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_chem-res-toxicol_19_6_16780356_s_8	16780356	4'F-DMA shows ligand binding affinity to  estrogen receptor (ER)alpha and ERbeta with similarity to both raloxifene  and to DMA.	bind
26897	3	8124	6	13	NULL	NULL	NULL	4'F-DMA	Chemical		has affinity for					ERbeta	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_chem-res-toxicol_19_6_16780356_s_8	16780356	4'F-DMA shows ligand binding affinity to  estrogen receptor (ER)alpha and ERbeta with similarity to both raloxifene  and to DMA.	bind
26898	4	8124	6	13	NULL	NULL	NULL	raloxifene	Chemical		has affinity for					ERalpha	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_chem-res-toxicol_19_6_16780356_s_8	16780356	4'F-DMA shows ligand binding affinity to  estrogen receptor (ER)alpha and ERbeta with similarity to both raloxifene  and to DMA.	bind
26899	5	8124	6	13	NULL	NULL	NULL	raloxifene	Chemical		has affinity for					ERbeta	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_chem-res-toxicol_19_6_16780356_s_8	16780356	4'F-DMA shows ligand binding affinity to  estrogen receptor (ER)alpha and ERbeta with similarity to both raloxifene  and to DMA.	bind
26900	6	8124	6	13	NULL	NULL	NULL	DMA	Chemical		has affinity for					ERalpha	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_chem-res-toxicol_19_6_16780356_s_8	16780356	4'F-DMA shows ligand binding affinity to  estrogen receptor (ER)alpha and ERbeta with similarity to both raloxifene  and to DMA.	bind
26901	7	8124	6	13	NULL	NULL	NULL	DMA	Chemical		has affinity for					ERbeta	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_chem-res-toxicol_19_6_16780356_s_8	16780356	4'F-DMA shows ligand binding affinity to  estrogen receptor (ER)alpha and ERbeta with similarity to both raloxifene  and to DMA.	bind
32366	1	8124	7	NULL	NULL	0	NULL	4'F-DMA	NULL		bind	NULL				ER alpha	NULL				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_chem-res-toxicol_19_6_16780356_s_8	16780356	4'F-DMA shows ligand binding affinity to  estrogen receptor (ER)alpha and ERbeta with similarity to both raloxifene  and to DMA.	bind
32367	2	8124	7	NULL	NULL	0	NULL	4'F-DMA	NULL		bind	NULL				ERbeta	NULL				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_chem-res-toxicol_19_6_16780356_s_8	16780356	4'F-DMA shows ligand binding affinity to  estrogen receptor (ER)alpha and ERbeta with similarity to both raloxifene  and to DMA.	bind
32368	3	8124	7	NULL	NULL	0	NULL	raloxifene	NULL		bind	NULL				ER alpha	NULL				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_chem-res-toxicol_19_6_16780356_s_8	16780356	4'F-DMA shows ligand binding affinity to  estrogen receptor (ER)alpha and ERbeta with similarity to both raloxifene  and to DMA.	bind
32369	4	8124	7	NULL	NULL	0	NULL	raloxifene	NULL		bind	NULL				ERbeta	NULL				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_chem-res-toxicol_19_6_16780356_s_8	16780356	4'F-DMA shows ligand binding affinity to  estrogen receptor (ER)alpha and ERbeta with similarity to both raloxifene  and to DMA.	bind
32370	5	8124	7	NULL	NULL	0	NULL	DMA	NULL		bind	NULL				ER alpha	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_chem-res-toxicol_19_6_16780356_s_8	16780356	4'F-DMA shows ligand binding affinity to  estrogen receptor (ER)alpha and ERbeta with similarity to both raloxifene  and to DMA.	bind
32371	6	8124	7	NULL	NULL	0	NULL	DMA	NULL		bind	NULL				ERbeta	NULL				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_chem-res-toxicol_19_6_16780356_s_8	16780356	4'F-DMA shows ligand binding affinity to  estrogen receptor (ER)alpha and ERbeta with similarity to both raloxifene  and to DMA.	bind
55836	7	8124	7	10	NULL	0	NULL	ER			is					estrogen receptor					NULL		0	NULL	NULL	NULL	abs-batch0700-0719_chem-res-toxicol_19_6_16780356_s_8	16780356	4'F-DMA shows ligand binding affinity to  estrogen receptor (ER)alpha and ERbeta with similarity to both raloxifene  and to DMA.	bind
26485	1	8125	6	13	NULL	NULL	NULL	EPOR	GP	soluble;; phosphorylated	bind			serine		JAK2	GP	genetically engineered			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_50_32430_s_155	8943308	4)  In vitro binding experiments showed that the soluble, serine-phosphorylated 78-kDa EPOR bound to genetically engineered JAK2 better than other forms of EPOR; however, EPO-induced tyrosine phosphorylation greatly increased the ability of the soluble, 78-kDa EPOR molecule to interact with immobilized JAK2.	bind
26486	2	8125	6	13	NULL	NULL	NULL	EPOR molecule	GP	soluble	interact with					JAK2	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_50_32430_s_155	8943308	4)  In vitro binding experiments showed that the soluble, serine-phosphorylated 78-kDa EPOR bound to genetically engineered JAK2 better than other forms of EPOR; however, EPO-induced tyrosine phosphorylation greatly increased the ability of the soluble, 78-kDa EPOR molecule to interact with immobilized JAK2.	bind
26487	3	8125	6	13	NULL	NULL	NULL	EPO 	GP		induces							phosphorylation of	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_50_32430_s_155	8943308	4)  In vitro binding experiments showed that the soluble, serine-phosphorylated 78-kDa EPOR bound to genetically engineered JAK2 better than other forms of EPOR; however, EPO-induced tyrosine phosphorylation greatly increased the ability of the soluble, 78-kDa EPOR molecule to interact with immobilized JAK2.	bind
26488	4	8125	6	13	NULL	NULL	NULL	statement 3	Process		increases					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_50_32430_s_155	8943308	4)  In vitro binding experiments showed that the soluble, serine-phosphorylated 78-kDa EPOR bound to genetically engineered JAK2 better than other forms of EPOR; however, EPO-induced tyrosine phosphorylation greatly increased the ability of the soluble, 78-kDa EPOR molecule to interact with immobilized JAK2.	bind
32372	1	8125	7	10	NULL	0	NULL	EPOR	NULL	soluble;;phosphorylated	bind	NULL		serine		JAK2	NULL	genetically engineered			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_50_32430_s_155	8943308	4)  In vitro binding experiments showed that the soluble, serine-phosphorylated 78-kDa EPOR bound to genetically engineered JAK2 better than other forms of EPOR; however, EPO-induced tyrosine phosphorylation greatly increased the ability of the soluble, 78-kDa EPOR molecule to interact with immobilized JAK2.	bind
32373	2	8125	7	NULL	NULL	0	NULL	EPOR	NULL		bind	NULL				JAK2	NULL	genetically engineered			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_50_32430_s_155	8943308	4)  In vitro binding experiments showed that the soluble, serine-phosphorylated 78-kDa EPOR bound to genetically engineered JAK2 better than other forms of EPOR; however, EPO-induced tyrosine phosphorylation greatly increased the ability of the soluble, 78-kDa EPOR molecule to interact with immobilized JAK2.	bind
32374	3	8125	7	NULL	NULL	0	NULL	EPOR	NULL		is a type of	NULL				78-kDa protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_50_32430_s_155	8943308	4)  In vitro binding experiments showed that the soluble, serine-phosphorylated 78-kDa EPOR bound to genetically engineered JAK2 better than other forms of EPOR; however, EPO-induced tyrosine phosphorylation greatly increased the ability of the soluble, 78-kDa EPOR molecule to interact with immobilized JAK2.	bind
32375	4	8125	7	NULL	NULL	0	NULL	statement 1	NULL	binding of	is better than 	NULL				statement 2	NULL	binding of			NULL	in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_271_50_32430_s_155	8943308	4)  In vitro binding experiments showed that the soluble, serine-phosphorylated 78-kDa EPOR bound to genetically engineered JAK2 better than other forms of EPOR; however, EPO-induced tyrosine phosphorylation greatly increased the ability of the soluble, 78-kDa EPOR molecule to interact with immobilized JAK2.	bind
32376	5	8125	7	NULL	NULL	0	NULL	EPOR molecule	NULL	soluble	interacts with	NULL				JAK2	NULL	immobilized			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_50_32430_s_155	8943308	4)  In vitro binding experiments showed that the soluble, serine-phosphorylated 78-kDa EPOR bound to genetically engineered JAK2 better than other forms of EPOR; however, EPO-induced tyrosine phosphorylation greatly increased the ability of the soluble, 78-kDa EPOR molecule to interact with immobilized JAK2.	bind
32377	6	8125	7	NULL	NULL	0	NULL	EPO	NULL		induce	NULL					NULL	phosphorylation of	tyrosine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_50_32430_s_155	8943308	4)  In vitro binding experiments showed that the soluble, serine-phosphorylated 78-kDa EPOR bound to genetically engineered JAK2 better than other forms of EPOR; however, EPO-induced tyrosine phosphorylation greatly increased the ability of the soluble, 78-kDa EPOR molecule to interact with immobilized JAK2.	bind
32378	7	8125	7	NULL	NULL	0	NULL	statement 6	NULL		increase	NULL	greatly			statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_50_32430_s_155	8943308	4)  In vitro binding experiments showed that the soluble, serine-phosphorylated 78-kDa EPOR bound to genetically engineered JAK2 better than other forms of EPOR; however, EPO-induced tyrosine phosphorylation greatly increased the ability of the soluble, 78-kDa EPOR molecule to interact with immobilized JAK2.	bind
26489	1	8126	6	13	NULL	NULL	NULL	Cas	GP	dominant-negative mutant	does not bind					Crk	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_16_11706_s_193	10766791	4) A dominant negative mutant of Cas which fails to bind Crk blocked H2O2-mediated activation of JNK but not ERK1/2 and p38.	bind
26490	2	8126	6	13	NULL	NULL	NULL	H2O2	Chemical		mediates					JNK	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_16_11706_s_193	10766791	4) A dominant negative mutant of Cas which fails to bind Crk blocked H2O2-mediated activation of JNK but not ERK1/2 and p38.	bind
26491	3	8126	6	13	NULL	NULL	NULL	Cas	GP	dominant-negative mutant	blocks					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_16_11706_s_193	10766791	4) A dominant negative mutant of Cas which fails to bind Crk blocked H2O2-mediated activation of JNK but not ERK1/2 and p38.	bind
26492	4	8126	6	13	NULL	NULL	NULL	H2O2	Chemical		mediates					Erk1/2	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_16_11706_s_193	10766791	4) A dominant negative mutant of Cas which fails to bind Crk blocked H2O2-mediated activation of JNK but not ERK1/2 and p38.	bind
26493	5	8126	6	13	NULL	NULL	NULL	H2O2	Chemical		mediates					p38	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_16_11706_s_193	10766791	4) A dominant negative mutant of Cas which fails to bind Crk blocked H2O2-mediated activation of JNK but not ERK1/2 and p38.	bind
26494	6	8126	6	13	NULL	NULL	NULL	Cas	GP	dominant-negative mutant	does not block					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_16_11706_s_193	10766791	4) A dominant negative mutant of Cas which fails to bind Crk blocked H2O2-mediated activation of JNK but not ERK1/2 and p38.	bind
26495	7	8126	6	13	NULL	NULL	NULL	Cas	GP	dominant-negative mutant	does not block					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_16_11706_s_193	10766791	4) A dominant negative mutant of Cas which fails to bind Crk blocked H2O2-mediated activation of JNK but not ERK1/2 and p38.	bind
32379	1	8126	7	NULL	NULL	0	NULL	Cas	NULL	dominant negative mutant	does not bind	NULL				Crk	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_16_11706_s_193	10766791	4) A dominant negative mutant of Cas which fails to bind Crk blocked H2O2-mediated activation of JNK but not ERK1/2 and p38.	bind
32380	2	8126	7	NULL	NULL	0	NULL	H2O2	NULL		mediates	NULL				JNK	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_16_11706_s_193	10766791	4) A dominant negative mutant of Cas which fails to bind Crk blocked H2O2-mediated activation of JNK but not ERK1/2 and p38.	bind
32381	3	8126	7	NULL	NULL	0	NULL	H2O2	NULL		mediates	NULL				ERK1/2	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_16_11706_s_193	10766791	4) A dominant negative mutant of Cas which fails to bind Crk blocked H2O2-mediated activation of JNK but not ERK1/2 and p38.	bind
32382	4	8126	7	NULL	NULL	0	NULL	H2O2	NULL		mediates	NULL				p38	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_16_11706_s_193	10766791	4) A dominant negative mutant of Cas which fails to bind Crk blocked H2O2-mediated activation of JNK but not ERK1/2 and p38.	bind
32383	5	8126	7	NULL	NULL	0	NULL	statement 1	NULL		blocks	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_16_11706_s_193	10766791	4) A dominant negative mutant of Cas which fails to bind Crk blocked H2O2-mediated activation of JNK but not ERK1/2 and p38.	bind
32384	6	8126	7	NULL	NULL	0	NULL	statement 1	NULL		does not block	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_16_11706_s_193	10766791	4) A dominant negative mutant of Cas which fails to bind Crk blocked H2O2-mediated activation of JNK but not ERK1/2 and p38.	bind
32385	7	8126	7	NULL	NULL	0	NULL	statement 1	NULL		does not block	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_16_11706_s_193	10766791	4) A dominant negative mutant of Cas which fails to bind Crk blocked H2O2-mediated activation of JNK but not ERK1/2 and p38.	bind
26496	1	8127	6	13	NULL	NULL	NULL	calcineurin/calmodulin	GP	activated	bind					FKBP12/TRPC6 anchor	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_32035_s_428	15994335	4) Activated calcineurin/calmodulin binds to the FKBP12/TRPC6 anchor, either before or after calcineurin dephosphorylates the channels.	bind
26497	2	8127	6	13	NULL	NULL	NULL	calcineurin	GP		dephosphorylates					channels	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_32035_s_428	15994335	4) Activated calcineurin/calmodulin binds to the FKBP12/TRPC6 anchor, either before or after calcineurin dephosphorylates the channels.	bind
32386	1	8127	7	NULL	NULL	0	NULL	calcineurin/calmodulin	NULL	activated	binds to	NULL				FKBP12/TRPC6 anchor	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_36_32035_s_428	15994335	4) Activated calcineurin/calmodulin binds to the FKBP12/TRPC6 anchor, either before or after calcineurin dephosphorylates the channels.	bind
32387	2	8127	7	NULL	NULL	0	NULL	calcineurin	NULL		dephosphorylates	NULL				channels	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_36_32035_s_428	15994335	4) Activated calcineurin/calmodulin binds to the FKBP12/TRPC6 anchor, either before or after calcineurin dephosphorylates the channels.	bind
26902	1	8128	6	13	NULL	NULL	NULL	Gbeta	GP		associates with					CCT/TRiC	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_29_20221_s_336	16702223	4) Addition of Ggamma to previously synthesized Gbeta under conditions allowing dimer formation ( Fig. 1) reduces Gbeta association with CCT/TRiC ( Fig. 10), indicating that Gbeta bound to CCT/TRiC is capable of functionally interacting with Ggamma and that exposure of the complex to Ggamma results in release of Gbeta from CCT/TRiC.	bind
26903	2	8128	6	13	NULL	NULL	NULL	statement 1	GP		interacts with		functionaly			Ggamma	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_29_20221_s_336	16702223	4) Addition of Ggamma to previously synthesized Gbeta under conditions allowing dimer formation ( Fig. 1) reduces Gbeta association with CCT/TRiC ( Fig. 10), indicating that Gbeta bound to CCT/TRiC is capable of functionally interacting with Ggamma and that exposure of the complex to Ggamma results in release of Gbeta from CCT/TRiC.	bind
26904	4	8128	6	13	NULL	NULL	NULL	Ggamma	GP	addition of	leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_29_20221_s_336	16702223	4) Addition of Ggamma to previously synthesized Gbeta under conditions allowing dimer formation ( Fig. 1) reduces Gbeta association with CCT/TRiC ( Fig. 10), indicating that Gbeta bound to CCT/TRiC is capable of functionally interacting with Ggamma and that exposure of the complex to Ggamma results in release of Gbeta from CCT/TRiC.	bind
46567	3	8128	6	13	NULL	NULL	NULL	Gbeta	GP		is released from					CCT/TRiC	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_29_20221_s_336	16702223	4) Addition of Ggamma to previously synthesized Gbeta under conditions allowing dimer formation ( Fig. 1) reduces Gbeta association with CCT/TRiC ( Fig. 10), indicating that Gbeta bound to CCT/TRiC is capable of functionally interacting with Ggamma and that exposure of the complex to Ggamma results in release of Gbeta from CCT/TRiC.	bind
32459	1	8128	7	NULL	NULL	0	NULL	Gbeta	NULL		associate with	NULL				CCT/TRiC	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_29_20221_s_336	16702223	4) Addition of Ggamma to previously synthesized Gbeta under conditions allowing dimer formation ( Fig. 1) reduces Gbeta association with CCT/TRiC ( Fig. 10), indicating that Gbeta bound to CCT/TRiC is capable of functionally interacting with Ggamma and that exposure of the complex to Ggamma results in release of Gbeta from CCT/TRiC.	bind
32460	2	8128	7	NULL	NULL	0	NULL	Gbeta 	NULL		bind	NULL				CCT/TRiC	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_29_20221_s_336	16702223	4) Addition of Ggamma to previously synthesized Gbeta under conditions allowing dimer formation ( Fig. 1) reduces Gbeta association with CCT/TRiC ( Fig. 10), indicating that Gbeta bound to CCT/TRiC is capable of functionally interacting with Ggamma and that exposure of the complex to Ggamma results in release of Gbeta from CCT/TRiC.	bind
32461	3	8128	7	NULL	NULL	0	NULL	statement 2	NULL		interacts with	NULL				Ggamma	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_29_20221_s_336	16702223	4) Addition of Ggamma to previously synthesized Gbeta under conditions allowing dimer formation ( Fig. 1) reduces Gbeta association with CCT/TRiC ( Fig. 10), indicating that Gbeta bound to CCT/TRiC is capable of functionally interacting with Ggamma and that exposure of the complex to Ggamma results in release of Gbeta from CCT/TRiC.	bind
32462	4	8128	7	10	NULL	0	NULL	statement 3	NULL	exposure of	leads to	NULL				statement 7	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_29_20221_s_336	16702223	4) Addition of Ggamma to previously synthesized Gbeta under conditions allowing dimer formation ( Fig. 1) reduces Gbeta association with CCT/TRiC ( Fig. 10), indicating that Gbeta bound to CCT/TRiC is capable of functionally interacting with Ggamma and that exposure of the complex to Ggamma results in release of Gbeta from CCT/TRiC.	bind
32463	5	8128	7	NULL	NULL	0	NULL	Ggamma	NULL	addition of	allows	NULL				dimer	NULL	formation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_29_20221_s_336	16702223	4) Addition of Ggamma to previously synthesized Gbeta under conditions allowing dimer formation ( Fig. 1) reduces Gbeta association with CCT/TRiC ( Fig. 10), indicating that Gbeta bound to CCT/TRiC is capable of functionally interacting with Ggamma and that exposure of the complex to Ggamma results in release of Gbeta from CCT/TRiC.	bind
32464	6	8128	7	NULL	NULL	0	NULL	statement 5	NULL		reduces	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_29_20221_s_336	16702223	4) Addition of Ggamma to previously synthesized Gbeta under conditions allowing dimer formation ( Fig. 1) reduces Gbeta association with CCT/TRiC ( Fig. 10), indicating that Gbeta bound to CCT/TRiC is capable of functionally interacting with Ggamma and that exposure of the complex to Ggamma results in release of Gbeta from CCT/TRiC.	bind
46568	7	8128	7	10	NULL	0	NULL	Gbeta	NULL		is released from	NULL				CCT/TRiC	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_29_20221_s_336	16702223	4) Addition of Ggamma to previously synthesized Gbeta under conditions allowing dimer formation ( Fig. 1) reduces Gbeta association with CCT/TRiC ( Fig. 10), indicating that Gbeta bound to CCT/TRiC is capable of functionally interacting with Ggamma and that exposure of the complex to Ggamma results in release of Gbeta from CCT/TRiC.	bind
26498	1	8129	6	13	NULL	NULL	NULL	AKT	GP		phosphorylates					p21Cip1	GP				NULL	HER-2/ neu-overexpressing cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_9684_s_176	11779850	4) AKT directly phosphorylates p21Cip1 in HER-2/ neu-overexpressing ( 14) as well as in native human endothelial cells ( 9), and 5) AKT phosphorylation regulates p21Cip1 binding to PCNA ( 9).	bind
26499	2	8129	6	13	NULL	NULL	NULL	AKT	GP		phosphorylates		directly			p21Cip1	GP				NULL	native human endothelial cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_9684_s_176	11779850	4) AKT directly phosphorylates p21Cip1 in HER-2/ neu-overexpressing ( 14) as well as in native human endothelial cells ( 9), and 5) AKT phosphorylation regulates p21Cip1 binding to PCNA ( 9).	bind
26500	3	8129	6	13	NULL	NULL	NULL	p21Cip1	GP		bind					PCNA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_9684_s_176	11779850	4) AKT directly phosphorylates p21Cip1 in HER-2/ neu-overexpressing ( 14) as well as in native human endothelial cells ( 9), and 5) AKT phosphorylation regulates p21Cip1 binding to PCNA ( 9).	bind
26501	4	8129	6	13	NULL	NULL	NULL	AKT	GP	phosphorylation of	regulates					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_9684_s_176	11779850	4) AKT directly phosphorylates p21Cip1 in HER-2/ neu-overexpressing ( 14) as well as in native human endothelial cells ( 9), and 5) AKT phosphorylation regulates p21Cip1 binding to PCNA ( 9).	bind
32465	1	8129	7	NULL	NULL	0	NULL	AKT	NULL		phosphorylates	NULL	directly			p21Cip1	NULL				NULL	HER-2/ neu-overexpressing cells	0	NULL	NULL	NULL	gw60_jbiolchem_277_12_9684_s_176	11779850	4) AKT directly phosphorylates p21Cip1 in HER-2/ neu-overexpressing ( 14) as well as in native human endothelial cells ( 9), and 5) AKT phosphorylation regulates p21Cip1 binding to PCNA ( 9).	bind
32466	2	8129	7	NULL	NULL	0	NULL	AKT	NULL		phosphorylates	NULL	directly			p21Cip1	NULL				NULL	native human endothelial cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_9684_s_176	11779850	4) AKT directly phosphorylates p21Cip1 in HER-2/ neu-overexpressing ( 14) as well as in native human endothelial cells ( 9), and 5) AKT phosphorylation regulates p21Cip1 binding to PCNA ( 9).	bind
32467	3	8129	7	NULL	NULL	0	NULL	 p21Cip1	NULL		bind	NULL				PCNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_12_9684_s_176	11779850	4) AKT directly phosphorylates p21Cip1 in HER-2/ neu-overexpressing ( 14) as well as in native human endothelial cells ( 9), and 5) AKT phosphorylation regulates p21Cip1 binding to PCNA ( 9).	bind
32468	4	8129	7	NULL	NULL	0	NULL	AKT	NULL	phosphorylation of	regulates	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_12_9684_s_176	11779850	4) AKT directly phosphorylates p21Cip1 in HER-2/ neu-overexpressing ( 14) as well as in native human endothelial cells ( 9), and 5) AKT phosphorylation regulates p21Cip1 binding to PCNA ( 9).	bind
26502	1	8130	6	13	NULL	NULL	NULL	actin	GP		bind								C domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_15_10589_s_311	16403731	4) Binding of actin and the Arp2/3 complex to the C domain is mutually exclusive.	bind
26503	2	8130	6	13	NULL	NULL	NULL	Arp2/3 complex	GP		bind								C domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_15_10589_s_311	16403731	4) Binding of actin and the Arp2/3 complex to the C domain is mutually exclusive.	bind
26504	3	8130	6	13	NULL	NULL	NULL	statement 1	Process		is independent of					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_15_10589_s_311	16403731	4) Binding of actin and the Arp2/3 complex to the C domain is mutually exclusive.	bind
32469	1	8130	7	NULL	NULL	0	NULL	actin	NULL		bind	NULL					NULL		C domain		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_15_10589_s_311	16403731	4) Binding of actin and the Arp2/3 complex to the C domain is mutually exclusive.	bind
32470	2	8130	7	NULL	NULL	0	NULL	Arp2/3 complex 	NULL		bind	NULL					NULL		C domain		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_15_10589_s_311	16403731	4) Binding of actin and the Arp2/3 complex to the C domain is mutually exclusive.	bind
32471	3	8130	7	NULL	NULL	0	NULL	statement 1	NULL		is mutually exclusive to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_15_10589_s_311	16403731	4) Binding of actin and the Arp2/3 complex to the C domain is mutually exclusive.	bind
26505	1	8131	6	13	NULL	NULL	NULL	Ggamma	GP		bind					Gbeta	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_31_22261_s_358	16717095	4) Ggamma binds Gbeta forming a PhLP.	bind
26506	2	8131	6	13	NULL	NULL	NULL	statement 1	GP		forms a					PhLP	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_31_22261_s_358	16717095	4) Ggamma binds Gbeta forming a PhLP.	bind
32472	1	8131	7	NULL	NULL	0	NULL	Ggamma	NULL		binds	NULL				Gbeta	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_31_22261_s_358	16717095	4) Ggamma binds Gbeta forming a PhLP.	bind
32473	2	8131	7	NULL	NULL	0	NULL	statement 1	NULL		forms	NULL				PhLP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_31_22261_s_358	16717095	4) Ggamma binds Gbeta forming a PhLP.	bind
26507	1	8132	6	13	NULL	NULL	NULL	Grb2	GP		bind					TrkA	GP				NULL	yeast	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_24_18225_s_237	10748052	4) Grb2 binding to TrkA in yeast is independent of Tyr499/Tyr679/Tyr794 but requires the activation loop tyrosines Tyr683/Tyr684.	bind
26508	2	8132	6	13	NULL	NULL	NULL	statement 1	Process		is independent of								Tyr499/Tyr679/Tyr794		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_24_18225_s_237	10748052	4) Grb2 binding to TrkA in yeast is independent of Tyr499/Tyr679/Tyr794 but requires the activation loop tyrosines Tyr683/Tyr684.	bind
26509	3	8132	6	13	NULL	NULL	NULL	statement 1	Process		requires					activation loop	GP		tyrosines Tyr683/Tyr684		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_24_18225_s_237	10748052	4) Grb2 binding to TrkA in yeast is independent of Tyr499/Tyr679/Tyr794 but requires the activation loop tyrosines Tyr683/Tyr684.	bind
32474	1	8132	7	NULL	NULL	0	NULL	Grb2	NULL		bind	NULL				 TrkA	NULL				NULL	yeast	0	NULL	NULL	NULL	gw60_jbiolchem_275_24_18225_s_237	10748052	4) Grb2 binding to TrkA in yeast is independent of Tyr499/Tyr679/Tyr794 but requires the activation loop tyrosines Tyr683/Tyr684.	bind
32475	2	8132	7	10	NULL	0	NULL	statement 1			is independent of								Tyr499/Tyr679/Tyr794		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_24_18225_s_237	10748052	4) Grb2 binding to TrkA in yeast is independent of Tyr499/Tyr679/Tyr794 but requires the activation loop tyrosines Tyr683/Tyr684.	bind
32476	3	8132	7	NULL	NULL	0	NULL	statement 2	NULL		requires	NULL				activation loop	NULL		tyrosines Tyr683/Tyr684		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_24_18225_s_237	10748052	4) Grb2 binding to TrkA in yeast is independent of Tyr499/Tyr679/Tyr794 but requires the activation loop tyrosines Tyr683/Tyr684.	bind
26510	1	8133	6	13	NULL	NULL	NULL	FKBP12	GP		bind					TRPC6A/B channels	GP	site immediately adjacent to	phosphoserine (768/714)		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_32035_s_349	15994335	4) Immunophilin FKBP12 binds to the TRPC6A/B channels at a site immediately adjacent  to the phosphoserine (768/714), creating a site for the binding of calcineurin/calmodulin.	bind
26511	2	8133	6	13	NULL	NULL	NULL	statement 1	Process		creates					calcineurin/calmodulin	GP	binding site for			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_32035_s_349	15994335	4) Immunophilin FKBP12 binds to the TRPC6A/B channels at a site immediately adjacent  to the phosphoserine (768/714), creating a site for the binding of calcineurin/calmodulin.	bind
46569	3	8133	6	13	NULL	NULL	NULL	FKBP12	GP		is a type of					immunophilin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_32035_s_349	15994335	4) Immunophilin FKBP12 binds to the TRPC6A/B channels at a site immediately adjacent  to the phosphoserine (768/714), creating a site for the binding of calcineurin/calmodulin.	bind
32477	1	8133	7	10	NULL	0	NULL	FKBP12 	NULL		binds to	NULL				TRPC6A/B channels	NULL	site adjacent to	phosphoserine (768/714)		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_32035_s_349	15994335	4) Immunophilin FKBP12 binds to the TRPC6A/B channels at a site immediately adjacent  to the phosphoserine (768/714), creating a site for the binding of calcineurin/calmodulin.	bind
32478	2	8133	7	10	NULL	0	NULL	statement 1	NULL		create	NULL				calcineurin/calmodulin	NULL	binding site for			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_32035_s_349	15994335	4) Immunophilin FKBP12 binds to the TRPC6A/B channels at a site immediately adjacent  to the phosphoserine (768/714), creating a site for the binding of calcineurin/calmodulin.	bind
46570	3	8133	7	10	NULL	0	NULL	FKBP12	NULL		is a type of	NULL				immunophilin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_36_32035_s_349	15994335	4) Immunophilin FKBP12 binds to the TRPC6A/B channels at a site immediately adjacent  to the phosphoserine (768/714), creating a site for the binding of calcineurin/calmodulin.	bind
26512	1	8134	6	13	NULL	NULL	NULL	Phosphatases	GP		dephosphorylate					phospholamban	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_52_33561_s_138	8969222	4) Phosphatases that dephosphorylate phospholamban could be inhibited by a PKA-dependent mechanism.	bind
26513	2	8134	6	13	NULL	NULL	NULL	statement 1	Process		is inhibited by					PKA-dependent mechanism	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_52_33561_s_138	8969222	4) Phosphatases that dephosphorylate phospholamban could be inhibited by a PKA-dependent mechanism.	bind
32479	1	8134	7	NULL	NULL	0	NULL	Phosphatases	NULL		dephosphorylate	NULL				phospholamban	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_52_33561_s_138	8969222	4) Phosphatases that dephosphorylate phospholamban could be inhibited by a PKA-dependent mechanism.	bind
32480	2	8134	7	NULL	NULL	0	NULL	PKA-dependent mechanism	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_52_33561_s_138	8969222	4) Phosphatases that dephosphorylate phospholamban could be inhibited by a PKA-dependent mechanism.	bind
26514	1	8135	6	13	NULL	NULL	NULL	gp180	GP	purified	bind					T cells	Cell	peripheral blood			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12786_s_10	9139738	4) Purified gp180 can bind to peripheral blood T cells and activate p56 lck. 5) gp180 can activate p56 lck in 3G8 (a murine T cell hybridoma transfected with human CD8alpha cDNA) but not in 3G4 (CD4 transfectant), suggesting that gp180 binds to CD8.	bind
26515	2	8135	6	13	NULL	NULL	NULL	statement 1	Process		activate					p56 lck	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12786_s_10	9139738	4) Purified gp180 can bind to peripheral blood T cells and activate p56 lck. 5) gp180 can activate p56 lck in 3G8 (a murine T cell hybridoma transfected with human CD8alpha cDNA) but not in 3G4 (CD4 transfectant), suggesting that gp180 binds to CD8.	bind
26516	3	8135	6	13	NULL	NULL	NULL	gp180	GP		bind					CD8	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12786_s_10	9139738	4) Purified gp180 can bind to peripheral blood T cells and activate p56 lck. 5) gp180 can activate p56 lck in 3G8 (a murine T cell hybridoma transfected with human CD8alpha cDNA) but not in 3G4 (CD4 transfectant), suggesting that gp180 binds to CD8.	bind
26517	4	8135	6	13	NULL	NULL	NULL	gp180	GP		activate					p56 lck	GP				NULL	3G8	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12786_s_10	9139738	4) Purified gp180 can bind to peripheral blood T cells and activate p56 lck. 5) gp180 can activate p56 lck in 3G8 (a murine T cell hybridoma transfected with human CD8alpha cDNA) but not in 3G4 (CD4 transfectant), suggesting that gp180 binds to CD8.	bind
26518	5	8135	6	13	NULL	NULL	NULL	T cell hybridoma	Cell	murine	transfected with					CD8alpha cDNA	NucleicAcid	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12786_s_10	9139738	4) Purified gp180 can bind to peripheral blood T cells and activate p56 lck. 5) gp180 can activate p56 lck in 3G8 (a murine T cell hybridoma transfected with human CD8alpha cDNA) but not in 3G4 (CD4 transfectant), suggesting that gp180 binds to CD8.	bind
26519	6	8135	6	13	NULL	NULL	NULL	3G8	Cell		is					statement 5	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12786_s_10	9139738	4) Purified gp180 can bind to peripheral blood T cells and activate p56 lck. 5) gp180 can activate p56 lck in 3G8 (a murine T cell hybridoma transfected with human CD8alpha cDNA) but not in 3G4 (CD4 transfectant), suggesting that gp180 binds to CD8.	bind
26520	7	8135	6	13	NULL	NULL	NULL	3G4	Cell		is a type of					CD4 transfectant	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12786_s_10	9139738	4) Purified gp180 can bind to peripheral blood T cells and activate p56 lck. 5) gp180 can activate p56 lck in 3G8 (a murine T cell hybridoma transfected with human CD8alpha cDNA) but not in 3G4 (CD4 transfectant), suggesting that gp180 binds to CD8.	bind
26521	8	8135	6	13	NULL	NULL	NULL	gp180	GP		does not activate					p56 lck	GP				NULL	3G4	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12786_s_10	9139738	4) Purified gp180 can bind to peripheral blood T cells and activate p56 lck. 5) gp180 can activate p56 lck in 3G8 (a murine T cell hybridoma transfected with human CD8alpha cDNA) but not in 3G4 (CD4 transfectant), suggesting that gp180 binds to CD8.	bind
26522	9	8135	6	13	NULL	NULL	NULL	statement 2	Process		suggests					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12786_s_10	9139738	4) Purified gp180 can bind to peripheral blood T cells and activate p56 lck. 5) gp180 can activate p56 lck in 3G8 (a murine T cell hybridoma transfected with human CD8alpha cDNA) but not in 3G4 (CD4 transfectant), suggesting that gp180 binds to CD8.	bind
32481	1	8135	7	10	NULL	0	NULL	gp180		purified	bind					T cells		 peripheral blood			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12786_s_10	9139738	4) Purified gp180 can bind to peripheral blood T cells and activate p56 lck. 5) gp180 can activate p56 lck in 3G8 (a murine T cell hybridoma transfected with human CD8alpha cDNA) but not in 3G4 (CD4 transfectant), suggesting that gp180 binds to CD8.	bind
32482	2	8135	7	NULL	NULL	0	NULL	statement 1	NULL		activates	NULL				p56 lck	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_19_12786_s_10	9139738	4) Purified gp180 can bind to peripheral blood T cells and activate p56 lck. 5) gp180 can activate p56 lck in 3G8 (a murine T cell hybridoma transfected with human CD8alpha cDNA) but not in 3G4 (CD4 transfectant), suggesting that gp180 binds to CD8.	bind
32483	3	8135	7	NULL	NULL	0	NULL	gp180	NULL		activate	NULL				p56 lck	NULL				NULL	3G8 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12786_s_10	9139738	4) Purified gp180 can bind to peripheral blood T cells and activate p56 lck. 5) gp180 can activate p56 lck in 3G8 (a murine T cell hybridoma transfected with human CD8alpha cDNA) but not in 3G4 (CD4 transfectant), suggesting that gp180 binds to CD8.	bind
32484	4	8135	7	NULL	NULL	0	NULL	gp 180	NULL		does not activate	NULL				p56 lck	NULL				NULL	3G4 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12786_s_10	9139738	4) Purified gp180 can bind to peripheral blood T cells and activate p56 lck. 5) gp180 can activate p56 lck in 3G8 (a murine T cell hybridoma transfected with human CD8alpha cDNA) but not in 3G4 (CD4 transfectant), suggesting that gp180 binds to CD8.	bind
32485	5	8135	7	NULL	NULL	0	NULL	gp180	NULL		binds to	NULL				CD8	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_19_12786_s_10	9139738	4) Purified gp180 can bind to peripheral blood T cells and activate p56 lck. 5) gp180 can activate p56 lck in 3G8 (a murine T cell hybridoma transfected with human CD8alpha cDNA) but not in 3G4 (CD4 transfectant), suggesting that gp180 binds to CD8.	bind
32486	6	8135	7	10	NULL	0	NULL	 3G8			is					statement 8					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12786_s_10	9139738	4) Purified gp180 can bind to peripheral blood T cells and activate p56 lck. 5) gp180 can activate p56 lck in 3G8 (a murine T cell hybridoma transfected with human CD8alpha cDNA) but not in 3G4 (CD4 transfectant), suggesting that gp180 binds to CD8.	bind
32487	7	8135	7	NULL	NULL	0	NULL	3G4	NULL		is a type of	NULL				CD4 transfectant	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_19_12786_s_10	9139738	4) Purified gp180 can bind to peripheral blood T cells and activate p56 lck. 5) gp180 can activate p56 lck in 3G8 (a murine T cell hybridoma transfected with human CD8alpha cDNA) but not in 3G4 (CD4 transfectant), suggesting that gp180 binds to CD8.	bind
46571	8	8135	7	10	NULL	0	NULL	T cell hybridoma	NULL	murine	is transfected with	NULL				CD8alpha cDNA	NULL	human			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_19_12786_s_10	9139738	4) Purified gp180 can bind to peripheral blood T cells and activate p56 lck. 5) gp180 can activate p56 lck in 3G8 (a murine T cell hybridoma transfected with human CD8alpha cDNA) but not in 3G4 (CD4 transfectant), suggesting that gp180 binds to CD8.	bind
26523	1	8136	6	13	NULL	NULL	NULL	MyoD	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_31_19140_s_318	9235903	4) S5a greatly enhanced the DNA binding of MyoD and E12 homodimers while having a less pronounced effect on MyoD-E12 heterodimers.	bind
26524	2	8136	6	13	NULL	NULL	NULL	E12 homodimers	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_31_19140_s_318	9235903	4) S5a greatly enhanced the DNA binding of MyoD and E12 homodimers while having a less pronounced effect on MyoD-E12 heterodimers.	bind
26525	3	8136	6	13	NULL	NULL	NULL	S5a	GP		enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_31_19140_s_318	9235903	4) S5a greatly enhanced the DNA binding of MyoD and E12 homodimers while having a less pronounced effect on MyoD-E12 heterodimers.	bind
26526	4	8136	6	13	NULL	NULL	NULL	S5a	GP		enhance					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_31_19140_s_318	9235903	4) S5a greatly enhanced the DNA binding of MyoD and E12 homodimers while having a less pronounced effect on MyoD-E12 heterodimers.	bind
26527	5	8136	6	13	NULL	NULL	NULL	S5a	GP		has less effect on					MyoD-E12 heterodimers	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_31_19140_s_318	9235903	4) S5a greatly enhanced the DNA binding of MyoD and E12 homodimers while having a less pronounced effect on MyoD-E12 heterodimers.	bind
32488	1	8136	7	NULL	NULL	0	NULL	MyoD	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_31_19140_s_318	9235903	4) S5a greatly enhanced the DNA binding of MyoD and E12 homodimers while having a less pronounced effect on MyoD-E12 heterodimers.	bind
32489	2	8136	7	NULL	NULL	0	NULL	E12 homodimers	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_31_19140_s_318	9235903	4) S5a greatly enhanced the DNA binding of MyoD and E12 homodimers while having a less pronounced effect on MyoD-E12 heterodimers.	bind
32490	3	8136	7	NULL	NULL	0	NULL	S5a	NULL		enhance	NULL	greatly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_31_19140_s_318	9235903	4) S5a greatly enhanced the DNA binding of MyoD and E12 homodimers while having a less pronounced effect on MyoD-E12 heterodimers.	bind
32491	4	8136	7	NULL	NULL	0	NULL	S5a	NULL		enhance	NULL	greatly			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_31_19140_s_318	9235903	4) S5a greatly enhanced the DNA binding of MyoD and E12 homodimers while having a less pronounced effect on MyoD-E12 heterodimers.	bind
32492	5	8136	7	NULL	NULL	0	NULL	S5a	NULL		less effect on	NULL				MyoD-E12 heterodimers	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_31_19140_s_318	9235903	4) S5a greatly enhanced the DNA binding of MyoD and E12 homodimers while having a less pronounced effect on MyoD-E12 heterodimers.	bind
26528	1	8137	6	13	NULL	NULL	NULL	HO-1	GP		bind			amino acids 0-117		HO-2	GP				NULL	brain homogenates	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_51_50999_s_215	14514669	4) The addition of a fragment necessary for HO-1 binding to HO-2 (amino acids 0-117 of HO-1) to the brain homogenates significantly reduced total HO activity of the complex (decreased to 0.23  plus-or-minus  0.03  versus 0.36  plus-or-minus  0.04 nmol CO/mg protein/h in samples incubated with 0-117 fragment  versus brain homogenates alone).	bind
32493	1	8137	7	10	NULL	0	NULL	 HO-1 			bind			amino acids 0-117		HO-2					NULL	brain homogenates	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_51_50999_s_215	14514669	4) The addition of a fragment necessary for HO-1 binding to HO-2 (amino acids 0-117 of HO-1) to the brain homogenates significantly reduced total HO activity of the complex (decreased to 0.23  plus-or-minus  0.03  versus 0.36  plus-or-minus  0.04 nmol CO/mg protein/h in samples incubated with 0-117 fragment  versus brain homogenates alone).	bind
26529	1	8138	6	13	NULL	NULL	NULL	p67 phox	GP		bind					p22 phox peptides	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_277_10_11733522_s_12	11733522	4) The binding affinity of p67(phox) for p22(phox) peptides is lower than  that of p47(phox).	bind
26530	2	8138	6	13	NULL	NULL	NULL	p47 phox	GP		bind					p22 phox peptides	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_277_10_11733522_s_12	11733522	4) The binding affinity of p67(phox) for p22(phox) peptides is lower than  that of p47(phox).	bind
26531	3	8138	6	13	NULL	NULL	NULL	statement 1	Process	affinity of	is lower than					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_277_10_11733522_s_12	11733522	4) The binding affinity of p67(phox) for p22(phox) peptides is lower than  that of p47(phox).	bind
32496	1	8138	7	NULL	NULL	0	NULL	 p67(phox)	NULL		bind	NULL				p22(phox) peptides	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_277_10_11733522_s_12	11733522	4) The binding affinity of p67(phox) for p22(phox) peptides is lower than  that of p47(phox).	bind
32497	2	8138	7	NULL	NULL	0	NULL	 p67(phox)	NULL		bind	NULL				p47(phox)	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_277_10_11733522_s_12	11733522	4) The binding affinity of p67(phox) for p22(phox) peptides is lower than  that of p47(phox).	bind
32498	3	8138	7	10	NULL	0	NULL	statement 1	NULL	affinity of	is lower than	NULL				statement 2	NULL	affinity of			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_277_10_11733522_s_12	11733522	4) The binding affinity of p67(phox) for p22(phox) peptides is lower than  that of p47(phox).	bind
26533	1	8139	6	13	NULL	NULL	NULL	InsP(3)R1 splice variant	GP		bind			SII(+) coupling domain		AKAP9	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0580-0599_j-biol-chem_279_18_14982933_s_15	14982933	4) The InsP(3)R association with AKAP9 is specific for  type 1 InsP(3)R. 5) Both the SII(+) and the SII(-) coupling domain splice  variants of InsP(3)R1 bind to AKAP9.	bind
26534	2	8139	6	13	NULL	NULL	NULL	InsP(3)R1 splice variant	GP		bind			SII(-) coupling domain		AKAP9	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0580-0599_j-biol-chem_279_18_14982933_s_15	14982933	4) The InsP(3)R association with AKAP9 is specific for  type 1 InsP(3)R. 5) Both the SII(+) and the SII(-) coupling domain splice  variants of InsP(3)R1 bind to AKAP9.	bind
55932	3	8139	6	13	NULL	NULL	NULL	InsP(3)R	GP		associate with					AKAP9	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0580-0599_j-biol-chem_279_18_14982933_s_15	14982933	4) The InsP(3)R association with AKAP9 is specific for  type 1 InsP(3)R. 5) Both the SII(+) and the SII(-) coupling domain splice  variants of InsP(3)R1 bind to AKAP9.	bind
55933	4	8139	6	13	NULL	NULL	NULL	statement 3	Process		is specific for					type 1 InsP(3)R	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0580-0599_j-biol-chem_279_18_14982933_s_15	14982933	4) The InsP(3)R association with AKAP9 is specific for  type 1 InsP(3)R. 5) Both the SII(+) and the SII(-) coupling domain splice  variants of InsP(3)R1 bind to AKAP9.	bind
32499	1	8139	7	NULL	NULL	0	NULL	 InsP(3)R	NULL		associate with	NULL				AKAP9	NULL				NULL		0	NULL	NULL	NULL	abs-batch0580-0599_j-biol-chem_279_18_14982933_s_15	14982933	4) The InsP(3)R association with AKAP9 is specific for  type 1 InsP(3)R. 5) Both the SII(+) and the SII(-) coupling domain splice  variants of InsP(3)R1 bind to AKAP9.	bind
32500	2	8139	7	NULL	NULL	0	NULL	statement 1	NULL		is specific for	NULL				type 1 InsP(3)R	NULL				NULL		0	NULL	NULL	NULL	abs-batch0580-0599_j-biol-chem_279_18_14982933_s_15	14982933	4) The InsP(3)R association with AKAP9 is specific for  type 1 InsP(3)R. 5) Both the SII(+) and the SII(-) coupling domain splice  variants of InsP(3)R1 bind to AKAP9.	bind
32501	3	8139	7	10	NULL	0	NULL	 InsP(3)R1 splice variant			binds to			 SII(+) coupling domain		AKAP9					NULL		NULL	NULL	NULL	NULL	abs-batch0580-0599_j-biol-chem_279_18_14982933_s_15	14982933	4) The InsP(3)R association with AKAP9 is specific for  type 1 InsP(3)R. 5) Both the SII(+) and the SII(-) coupling domain splice  variants of InsP(3)R1 bind to AKAP9.	bind
32502	4	8139	7	10	NULL	0	NULL	InsP(3)R1 splice variant			binds to			SII(-) coupling domain		AKAP9					NULL		NULL	NULL	NULL	NULL	abs-batch0580-0599_j-biol-chem_279_18_14982933_s_15	14982933	4) The InsP(3)R association with AKAP9 is specific for  type 1 InsP(3)R. 5) Both the SII(+) and the SII(-) coupling domain splice  variants of InsP(3)R1 bind to AKAP9.	bind
26535	1	8140	6	13	NULL	NULL	NULL	nNOS	GP		contains an			FMN-binding subdomain of the reductase domain		autoinhibitory loop	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_19_16888_s_215	11884406	4) There is an autoinhibitory loop in the FMN-binding subdomain of the reductase domain in nNOS and eNOS not present in iNOS ( 18,  27,  34-36).	bind
26536	2	8140	6	13	NULL	NULL	NULL	eNOS	GP		contains an			FMN-binding subdomain of the reductase domain		autoinhibitory loop	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_19_16888_s_215	11884406	4) There is an autoinhibitory loop in the FMN-binding subdomain of the reductase domain in nNOS and eNOS not present in iNOS ( 18,  27,  34-36).	bind
26537	3	8140	6	13	NULL	NULL	NULL	iNOS	GP		does not contain			FMN-binding subdomain of the reductase domain		autoinhibitory loop	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_19_16888_s_215	11884406	4) There is an autoinhibitory loop in the FMN-binding subdomain of the reductase domain in nNOS and eNOS not present in iNOS ( 18,  27,  34-36).	bind
32503	1	8140	7	10	NULL	0	NULL	autoinhibitory loop			is present in					nNOS			\tFMN-binding subdomain of the reductase domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_19_16888_s_215	11884406	4) There is an autoinhibitory loop in the FMN-binding subdomain of the reductase domain in nNOS and eNOS not present in iNOS ( 18,  27,  34-36).	bind
32504	2	8140	7	10	NULL	0	NULL	autoinhibitory loop			is present in					eNOS			\tFMN-binding subdomain of the reductase domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_19_16888_s_215	11884406	4) There is an autoinhibitory loop in the FMN-binding subdomain of the reductase domain in nNOS and eNOS not present in iNOS ( 18,  27,  34-36).	bind
32505	3	8140	7	10	NULL	0	NULL	autoinhibitory loop			is not present in					iNOS			\tFMN-binding subdomain of the reductase domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_19_16888_s_215	11884406	4) There is an autoinhibitory loop in the FMN-binding subdomain of the reductase domain in nNOS and eNOS not present in iNOS ( 18,  27,  34-36).	bind
26538	1	8141	6	13	NULL	NULL	NULL	Type 1 fimbriated E.coli	Organism		bind					THP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_13_9924_s_191	11134021	4) Type 1 fimbriated  E. coli binds equally well to THP and to bovine RNase B, the latter of which is known to possess a single high-mannose chain.	bind
26539	2	8141	6	13	NULL	NULL	NULL	Type 1 fimbriated E.coli	Organism		bind					RNase B	GP	bovine			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_13_9924_s_191	11134021	4) Type 1 fimbriated  E. coli binds equally well to THP and to bovine RNase B, the latter of which is known to possess a single high-mannose chain.	bind
26540	3	8141	6	13	NULL	NULL	NULL	statement 1	Process	affinity of	is equal to					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_13_9924_s_191	11134021	4) Type 1 fimbriated  E. coli binds equally well to THP and to bovine RNase B, the latter of which is known to possess a single high-mannose chain.	bind
26541	4	8141	6	13	NULL	NULL	NULL	RNase B	GP	bovine	possess								high-mannose chain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_13_9924_s_191	11134021	4) Type 1 fimbriated  E. coli binds equally well to THP and to bovine RNase B, the latter of which is known to possess a single high-mannose chain.	bind
32506	1	8141	7	NULL	NULL	0	NULL	Type 1 fimbriated E. coli 	NULL		binds	NULL				THP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_13_9924_s_191	11134021	4) Type 1 fimbriated  E. coli binds equally well to THP and to bovine RNase B, the latter of which is known to possess a single high-mannose chain.	bind
32507	2	8141	7	NULL	NULL	0	NULL	Type 1 fimbriated E. coli 	NULL		binds	NULL				RNase B	NULL	bovine			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_13_9924_s_191	11134021	4) Type 1 fimbriated  E. coli binds equally well to THP and to bovine RNase B, the latter of which is known to possess a single high-mannose chain.	bind
32508	3	8141	7	10	NULL	0	NULL	RNase B			possess								high-mannose chain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_13_9924_s_191	11134021	4) Type 1 fimbriated  E. coli binds equally well to THP and to bovine RNase B, the latter of which is known to possess a single high-mannose chain.	bind
55934	4	8141	7	10	NULL	0	NULL	statement 1		affinity of	is equal to					statement 2		affinity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_13_9924_s_191	11134021	4) Type 1 fimbriated  E. coli binds equally well to THP and to bovine RNase B, the latter of which is known to possess a single high-mannose chain.	bind
26542	1	8142	6	13	NULL	NULL	NULL	casein kinase II	GP		phosphorylates					IkappaBalpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29840_s_41	10882738	4) When compared with its unphosphorylated form, casein kinase II-phosphorylated IkappaBalpha binds the p50/p65 heterodimer and the p65 homodimer with 33- and 9-fold higher binding affinity, respectively.	bind
26543	2	8142	6	13	NULL	NULL	NULL	IkappaBalpha	GP	unphosphorylated	bind					p50/p65 heterodimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29840_s_41	10882738	4) When compared with its unphosphorylated form, casein kinase II-phosphorylated IkappaBalpha binds the p50/p65 heterodimer and the p65 homodimer with 33- and 9-fold higher binding affinity, respectively.	bind
26544	3	8142	6	13	NULL	NULL	NULL	IkappaBalpha	GP	unphosphorylated	bind					p65 homodimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29840_s_41	10882738	4) When compared with its unphosphorylated form, casein kinase II-phosphorylated IkappaBalpha binds the p50/p65 heterodimer and the p65 homodimer with 33- and 9-fold higher binding affinity, respectively.	bind
26608	4	8142	6	13	NULL	NULL	NULL	IkappaBalpha	GP	phosphorylated	bind					p50/p65 heterodimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29840_s_41	10882738	4) When compared with its unphosphorylated form, casein kinase II-phosphorylated IkappaBalpha binds the p50/p65 heterodimer and the p65 homodimer with 33- and 9-fold higher binding affinity, respectively.	bind
26609	5	8142	6	13	NULL	NULL	NULL	IkappaBalpha	GP	phosphorylated	bind					p65 homodimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29840_s_41	10882738	4) When compared with its unphosphorylated form, casein kinase II-phosphorylated IkappaBalpha binds the p50/p65 heterodimer and the p65 homodimer with 33- and 9-fold higher binding affinity, respectively.	bind
26610	6	8142	6	13	NULL	NULL	NULL	statement 4	Process	affinity of	is higher than					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29840_s_41	10882738	4) When compared with its unphosphorylated form, casein kinase II-phosphorylated IkappaBalpha binds the p50/p65 heterodimer and the p65 homodimer with 33- and 9-fold higher binding affinity, respectively.	bind
26611	7	8142	6	13	NULL	NULL	NULL	statement 5	Process	affinity of	is higher than					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29840_s_41	10882738	4) When compared with its unphosphorylated form, casein kinase II-phosphorylated IkappaBalpha binds the p50/p65 heterodimer and the p65 homodimer with 33- and 9-fold higher binding affinity, respectively.	bind
32509	1	8142	7	NULL	NULL	0	NULL	casein kinase II	NULL		phosphorylates	NULL				IkappaBalpha	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29840_s_41	10882738	4) When compared with its unphosphorylated form, casein kinase II-phosphorylated IkappaBalpha binds the p50/p65 heterodimer and the p65 homodimer with 33- and 9-fold higher binding affinity, respectively.	bind
32510	2	8142	7	NULL	NULL	0	NULL	statement 1	NULL		binds	NULL				p50/p65 heterodimer	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29840_s_41	10882738	4) When compared with its unphosphorylated form, casein kinase II-phosphorylated IkappaBalpha binds the p50/p65 heterodimer and the p65 homodimer with 33- and 9-fold higher binding affinity, respectively.	bind
32511	3	8142	7	NULL	NULL	0	NULL	statement 1	NULL		binds	NULL				p65 homodimer 	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29840_s_41	10882738	4) When compared with its unphosphorylated form, casein kinase II-phosphorylated IkappaBalpha binds the p50/p65 heterodimer and the p65 homodimer with 33- and 9-fold higher binding affinity, respectively.	bind
32512	4	8142	7	NULL	NULL	0	NULL	IkappaBalpha	NULL	unphosphorylated	binds	NULL				p50/p65 heterodimer	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29840_s_41	10882738	4) When compared with its unphosphorylated form, casein kinase II-phosphorylated IkappaBalpha binds the p50/p65 heterodimer and the p65 homodimer with 33- and 9-fold higher binding affinity, respectively.	bind
32513	5	8142	7	NULL	NULL	0	NULL	IkappaBalpha	NULL	unphosphorylated	binds	NULL				p65 homodimer	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29840_s_41	10882738	4) When compared with its unphosphorylated form, casein kinase II-phosphorylated IkappaBalpha binds the p50/p65 heterodimer and the p65 homodimer with 33- and 9-fold higher binding affinity, respectively.	bind
32514	6	8142	7	10	NULL	0	NULL	statement 2	NULL	affinity of	is higher than	NULL				statement 4	NULL	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29840_s_41	10882738	4) When compared with its unphosphorylated form, casein kinase II-phosphorylated IkappaBalpha binds the p50/p65 heterodimer and the p65 homodimer with 33- and 9-fold higher binding affinity, respectively.	bind
32515	7	8142	7	10	NULL	0	NULL	statement 3	NULL	affinity of	is higher than	NULL				statement 5	NULL	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29840_s_41	10882738	4) When compared with its unphosphorylated form, casein kinase II-phosphorylated IkappaBalpha binds the p50/p65 heterodimer and the p65 homodimer with 33- and 9-fold higher binding affinity, respectively.	bind
26612	1	8143	6	13	NULL	NULL	NULL	SHP-2	GP		bind					IRS-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_7_1081_s_104	12117720	4, 23 SHP2 also binds to IRS-1, 7 as do other adapter proteins.	bind
26613	2	8143	6	13	NULL	NULL	NULL	Adaptor proteins	GP		bind					IRS-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_7_1081_s_104	12117720	4, 23 SHP2 also binds to IRS-1, 7 as do other adapter proteins.	bind
32516	1	8143	7	NULL	NULL	0	NULL	 SHP2	NULL		binds to	NULL				IRS-1, 7	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_7_1081_s_104	12117720	4, 23 SHP2 also binds to IRS-1, 7 as do other adapter proteins.	bind
32517	2	8143	7	NULL	NULL	0	NULL	adapter proteins	NULL		binds to	NULL				IRS-1, 7	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_7_1081_s_104	12117720	4, 23 SHP2 also binds to IRS-1, 7 as do other adapter proteins.	bind
26614	1	8144	6	13	NULL	NULL	NULL	ASK1	GP		bind			C-terminal domain					TRAF domain		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1259_s_21	12089063	4, 5, 9, 10 The C-terminal domain of ASK1 binds to the TRAF-domain and this association is required for ASK1 activation by cytokines.	bind
26615	2	8144	6	13	NULL	NULL	NULL	cytokines	GP		activate					ASK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1259_s_21	12089063	4, 5, 9, 10 The C-terminal domain of ASK1 binds to the TRAF-domain and this association is required for ASK1 activation by cytokines.	bind
26616	3	8144	6	13	NULL	NULL	NULL	statement 1	Process		is required for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1259_s_21	12089063	4, 5, 9, 10 The C-terminal domain of ASK1 binds to the TRAF-domain and this association is required for ASK1 activation by cytokines.	bind
32518	1	8144	7	NULL	NULL	0	NULL	ASK1	NULL		binds to	NULL		C-terminal domain 			NULL		TRAF-domain		NULL		0	NULL	NULL	NULL	gw60_circulationres_90_12_1259_s_21	12089063	4, 5, 9, 10 The C-terminal domain of ASK1 binds to the TRAF-domain and this association is required for ASK1 activation by cytokines.	bind
32519	2	8144	7	NULL	NULL	0	NULL	cytokines	NULL		activates	NULL				ASK1 	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_12_1259_s_21	12089063	4, 5, 9, 10 The C-terminal domain of ASK1 binds to the TRAF-domain and this association is required for ASK1 activation by cytokines.	bind
32520	3	8144	7	NULL	NULL	0	NULL	statement 1	NULL		is required for	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_12_1259_s_21	12089063	4, 5, 9, 10 The C-terminal domain of ASK1 binds to the TRAF-domain and this association is required for ASK1 activation by cytokines.	bind
26617	1	8145	6	13	NULL	NULL	NULL	HDL	GP		bind					ECM	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1333_s_170	12089072	4, 8 Therefore, this further supports the idea that apo E is the principal determinant of HDL binding to the ECM via its binding to matrix proteoglycans.	bind
26618	2	8145	6	13	NULL	NULL	NULL	apoE	GP		bind					matrix proteoglycans	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1333_s_170	12089072	4, 8 Therefore, this further supports the idea that apo E is the principal determinant of HDL binding to the ECM via its binding to matrix proteoglycans.	bind
26619	3	8145	6	13	NULL	NULL	NULL	statement 2	Process		is the determinant		principal			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1333_s_170	12089072	4, 8 Therefore, this further supports the idea that apo E is the principal determinant of HDL binding to the ECM via its binding to matrix proteoglycans.	bind
32521	1	8145	7	NULL	NULL	0	NULL	HDL	NULL		binds	NULL				ECM	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1333_s_170	12089072	4, 8 Therefore, this further supports the idea that apo E is the principal determinant of HDL binding to the ECM via its binding to matrix proteoglycans.	bind
32522	2	8145	7	NULL	NULL	0	NULL	apo E	NULL		binds	NULL				matrix proteoglycans	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_12_1333_s_170	12089072	4, 8 Therefore, this further supports the idea that apo E is the principal determinant of HDL binding to the ECM via its binding to matrix proteoglycans.	bind
32523	3	8145	7	10	NULL	0	NULL	statement 2	NULL		is the determinant of	NULL	principal			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_12_1333_s_170	12089072	4, 8 Therefore, this further supports the idea that apo E is the principal determinant of HDL binding to the ECM via its binding to matrix proteoglycans.	bind
26620	1	8146	6	13	NULL	NULL	NULL	CCR3	GP		bind					CCL8	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1211_s_29	15130922	4,14 - 16    In addition to being the major receptor for CCL11, CCR3 also binds to CCL8 (MCP2), CCL7 (MCP3), CCL13 (MCP4), CCL5 (RANTES), CCL24 (eotaxin-2), CCL26 (eotaxin-3), and CCL15 (MIP5).	bind
26621	2	8146	6	13	NULL	NULL	NULL	CCR3	GP		bind					CCL7	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1211_s_29	15130922	4,14 - 16    In addition to being the major receptor for CCL11, CCR3 also binds to CCL8 (MCP2), CCL7 (MCP3), CCL13 (MCP4), CCL5 (RANTES), CCL24 (eotaxin-2), CCL26 (eotaxin-3), and CCL15 (MIP5).	bind
26622	3	8146	6	13	NULL	NULL	NULL	CCR3	GP		bind					CCL13	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1211_s_29	15130922	4,14 - 16    In addition to being the major receptor for CCL11, CCR3 also binds to CCL8 (MCP2), CCL7 (MCP3), CCL13 (MCP4), CCL5 (RANTES), CCL24 (eotaxin-2), CCL26 (eotaxin-3), and CCL15 (MIP5).	bind
26623	4	8146	6	13	NULL	NULL	NULL	CCR3	GP		bind					CCL5	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1211_s_29	15130922	4,14 - 16    In addition to being the major receptor for CCL11, CCR3 also binds to CCL8 (MCP2), CCL7 (MCP3), CCL13 (MCP4), CCL5 (RANTES), CCL24 (eotaxin-2), CCL26 (eotaxin-3), and CCL15 (MIP5).	bind
26624	5	8146	6	13	NULL	NULL	NULL	CCR3	GP		bind					CCL24	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1211_s_29	15130922	4,14 - 16    In addition to being the major receptor for CCL11, CCR3 also binds to CCL8 (MCP2), CCL7 (MCP3), CCL13 (MCP4), CCL5 (RANTES), CCL24 (eotaxin-2), CCL26 (eotaxin-3), and CCL15 (MIP5).	bind
26625	6	8146	6	13	NULL	NULL	NULL	CCR3	GP		bind					CCL26	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1211_s_29	15130922	4,14 - 16    In addition to being the major receptor for CCL11, CCR3 also binds to CCL8 (MCP2), CCL7 (MCP3), CCL13 (MCP4), CCL5 (RANTES), CCL24 (eotaxin-2), CCL26 (eotaxin-3), and CCL15 (MIP5).	bind
26626	7	8146	6	13	NULL	NULL	NULL	CCR3	GP		bind					CCL15	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1211_s_29	15130922	4,14 - 16    In addition to being the major receptor for CCL11, CCR3 also binds to CCL8 (MCP2), CCL7 (MCP3), CCL13 (MCP4), CCL5 (RANTES), CCL24 (eotaxin-2), CCL26 (eotaxin-3), and CCL15 (MIP5).	bind
26627	8	8146	6	13	NULL	NULL	NULL	CCR3	GP		bind					CCL11	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1211_s_29	15130922	4,14 - 16    In addition to being the major receptor for CCL11, CCR3 also binds to CCL8 (MCP2), CCL7 (MCP3), CCL13 (MCP4), CCL5 (RANTES), CCL24 (eotaxin-2), CCL26 (eotaxin-3), and CCL15 (MIP5).	bind
55935	9	8146	6	13	NULL	NULL	NULL	CCL8	GP		is					MCP2	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1211_s_29	15130922	4,14 - 16    In addition to being the major receptor for CCL11, CCR3 also binds to CCL8 (MCP2), CCL7 (MCP3), CCL13 (MCP4), CCL5 (RANTES), CCL24 (eotaxin-2), CCL26 (eotaxin-3), and CCL15 (MIP5).	bind
55936	10	8146	6	13	NULL	NULL	NULL	CCL7	GP		is					MCP3	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1211_s_29	15130922	4,14 - 16    In addition to being the major receptor for CCL11, CCR3 also binds to CCL8 (MCP2), CCL7 (MCP3), CCL13 (MCP4), CCL5 (RANTES), CCL24 (eotaxin-2), CCL26 (eotaxin-3), and CCL15 (MIP5).	bind
55937	11	8146	6	13	NULL	NULL	NULL	CCL13	GP		is					MCP4	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1211_s_29	15130922	4,14 - 16    In addition to being the major receptor for CCL11, CCR3 also binds to CCL8 (MCP2), CCL7 (MCP3), CCL13 (MCP4), CCL5 (RANTES), CCL24 (eotaxin-2), CCL26 (eotaxin-3), and CCL15 (MIP5).	bind
55938	12	8146	6	13	NULL	NULL	NULL	CCL5	GP		is					RANTES	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1211_s_29	15130922	4,14 - 16    In addition to being the major receptor for CCL11, CCR3 also binds to CCL8 (MCP2), CCL7 (MCP3), CCL13 (MCP4), CCL5 (RANTES), CCL24 (eotaxin-2), CCL26 (eotaxin-3), and CCL15 (MIP5).	bind
55939	13	8146	6	13	NULL	NULL	NULL	CCL24	GP		is					eotaxin-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1211_s_29	15130922	4,14 - 16    In addition to being the major receptor for CCL11, CCR3 also binds to CCL8 (MCP2), CCL7 (MCP3), CCL13 (MCP4), CCL5 (RANTES), CCL24 (eotaxin-2), CCL26 (eotaxin-3), and CCL15 (MIP5).	bind
55940	14	8146	6	13	NULL	NULL	NULL	CCL26	GP		is					eotaxin-3	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1211_s_29	15130922	4,14 - 16    In addition to being the major receptor for CCL11, CCR3 also binds to CCL8 (MCP2), CCL7 (MCP3), CCL13 (MCP4), CCL5 (RANTES), CCL24 (eotaxin-2), CCL26 (eotaxin-3), and CCL15 (MIP5).	bind
55941	15	8146	6	13	NULL	NULL	NULL	CCL15	GP		is					MIP5	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1211_s_29	15130922	4,14 - 16    In addition to being the major receptor for CCL11, CCR3 also binds to CCL8 (MCP2), CCL7 (MCP3), CCL13 (MCP4), CCL5 (RANTES), CCL24 (eotaxin-2), CCL26 (eotaxin-3), and CCL15 (MIP5).	bind
32596	1	8146	7	NULL	NULL	0	NULL	CCR3 	NULL		binds	NULL				CCL11	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1211_s_29	15130922	4,14 - 16    In addition to being the major receptor for CCL11, CCR3 also binds to CCL8 (MCP2), CCL7 (MCP3), CCL13 (MCP4), CCL5 (RANTES), CCL24 (eotaxin-2), CCL26 (eotaxin-3), and CCL15 (MIP5).	bind
32597	2	8146	7	NULL	NULL	0	NULL	CCR3	NULL		binds	NULL				CCL8	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1211_s_29	15130922	4,14 - 16    In addition to being the major receptor for CCL11, CCR3 also binds to CCL8 (MCP2), CCL7 (MCP3), CCL13 (MCP4), CCL5 (RANTES), CCL24 (eotaxin-2), CCL26 (eotaxin-3), and CCL15 (MIP5).	bind
32598	3	8146	7	NULL	NULL	0	NULL	CCR3	NULL		binds	NULL				CCL7	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1211_s_29	15130922	4,14 - 16    In addition to being the major receptor for CCL11, CCR3 also binds to CCL8 (MCP2), CCL7 (MCP3), CCL13 (MCP4), CCL5 (RANTES), CCL24 (eotaxin-2), CCL26 (eotaxin-3), and CCL15 (MIP5).	bind
32599	4	8146	7	NULL	NULL	0	NULL	CCR3 	NULL		binds	NULL				CCL13	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1211_s_29	15130922	4,14 - 16    In addition to being the major receptor for CCL11, CCR3 also binds to CCL8 (MCP2), CCL7 (MCP3), CCL13 (MCP4), CCL5 (RANTES), CCL24 (eotaxin-2), CCL26 (eotaxin-3), and CCL15 (MIP5).	bind
32600	5	8146	7	NULL	NULL	0	NULL	CCR3	NULL		binds	NULL				 CCL5	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1211_s_29	15130922	4,14 - 16    In addition to being the major receptor for CCL11, CCR3 also binds to CCL8 (MCP2), CCL7 (MCP3), CCL13 (MCP4), CCL5 (RANTES), CCL24 (eotaxin-2), CCL26 (eotaxin-3), and CCL15 (MIP5).	bind
32601	6	8146	7	NULL	NULL	0	NULL	CCR3	NULL		binds	NULL				CCL24	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1211_s_29	15130922	4,14 - 16    In addition to being the major receptor for CCL11, CCR3 also binds to CCL8 (MCP2), CCL7 (MCP3), CCL13 (MCP4), CCL5 (RANTES), CCL24 (eotaxin-2), CCL26 (eotaxin-3), and CCL15 (MIP5).	bind
32602	7	8146	7	NULL	NULL	0	NULL	CCR3	NULL		binds	NULL				CCL26	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1211_s_29	15130922	4,14 - 16    In addition to being the major receptor for CCL11, CCR3 also binds to CCL8 (MCP2), CCL7 (MCP3), CCL13 (MCP4), CCL5 (RANTES), CCL24 (eotaxin-2), CCL26 (eotaxin-3), and CCL15 (MIP5).	bind
32603	8	8146	7	NULL	NULL	0	NULL	CCR3	NULL		binds	NULL				CCL15	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1211_s_29	15130922	4,14 - 16    In addition to being the major receptor for CCL11, CCR3 also binds to CCL8 (MCP2), CCL7 (MCP3), CCL13 (MCP4), CCL5 (RANTES), CCL24 (eotaxin-2), CCL26 (eotaxin-3), and CCL15 (MIP5).	bind
32604	9	8146	7	NULL	NULL	0	NULL	CCL8	NULL		is	NULL				MCP2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1211_s_29	15130922	4,14 - 16    In addition to being the major receptor for CCL11, CCR3 also binds to CCL8 (MCP2), CCL7 (MCP3), CCL13 (MCP4), CCL5 (RANTES), CCL24 (eotaxin-2), CCL26 (eotaxin-3), and CCL15 (MIP5).	bind
32605	10	8146	7	NULL	NULL	0	NULL	CCL7	NULL		is	NULL				MCP3	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1211_s_29	15130922	4,14 - 16    In addition to being the major receptor for CCL11, CCR3 also binds to CCL8 (MCP2), CCL7 (MCP3), CCL13 (MCP4), CCL5 (RANTES), CCL24 (eotaxin-2), CCL26 (eotaxin-3), and CCL15 (MIP5).	bind
32606	11	8146	7	NULL	NULL	0	NULL	CCL13 	NULL		is	NULL				MCP4	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1211_s_29	15130922	4,14 - 16    In addition to being the major receptor for CCL11, CCR3 also binds to CCL8 (MCP2), CCL7 (MCP3), CCL13 (MCP4), CCL5 (RANTES), CCL24 (eotaxin-2), CCL26 (eotaxin-3), and CCL15 (MIP5).	bind
32607	12	8146	7	NULL	NULL	0	NULL	CCL5	NULL		is	NULL				RANTES	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1211_s_29	15130922	4,14 - 16    In addition to being the major receptor for CCL11, CCR3 also binds to CCL8 (MCP2), CCL7 (MCP3), CCL13 (MCP4), CCL5 (RANTES), CCL24 (eotaxin-2), CCL26 (eotaxin-3), and CCL15 (MIP5).	bind
32608	13	8146	7	NULL	NULL	0	NULL	CCL24	NULL		is	NULL				eotaxin-2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1211_s_29	15130922	4,14 - 16    In addition to being the major receptor for CCL11, CCR3 also binds to CCL8 (MCP2), CCL7 (MCP3), CCL13 (MCP4), CCL5 (RANTES), CCL24 (eotaxin-2), CCL26 (eotaxin-3), and CCL15 (MIP5).	bind
32609	14	8146	7	NULL	NULL	0	NULL	CCL26 	NULL		is	NULL				eotaxin-3	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1211_s_29	15130922	4,14 - 16    In addition to being the major receptor for CCL11, CCR3 also binds to CCL8 (MCP2), CCL7 (MCP3), CCL13 (MCP4), CCL5 (RANTES), CCL24 (eotaxin-2), CCL26 (eotaxin-3), and CCL15 (MIP5).	bind
32610	15	8146	7	NULL	NULL	0	NULL	CCL15	NULL		is	NULL				MIP5	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1211_s_29	15130922	4,14 - 16    In addition to being the major receptor for CCL11, CCR3 also binds to CCL8 (MCP2), CCL7 (MCP3), CCL13 (MCP4), CCL5 (RANTES), CCL24 (eotaxin-2), CCL26 (eotaxin-3), and CCL15 (MIP5).	bind
26681	1	8147	6	13	NULL	NULL	NULL	AMP	Chemical		bind					AMPK	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_4_323_s_133	16051890	4,21  It has been proposed that the binding of AMP to the AMPK makes it a better substrate whereas the binding of ATP makes it a poor substrate for the upstream kinase.	bind
26682	2	8147	6	13	NULL	NULL	NULL	ATP	Chemical		bind					AMPK	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_4_323_s_133	16051890	4,21  It has been proposed that the binding of AMP to the AMPK makes it a better substrate whereas the binding of ATP makes it a poor substrate for the upstream kinase.	bind
26906	3	8147	6	13	NULL	NULL	NULL	AMPK	GP		substrate for					upstream kinase	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_4_323_s_133	16051890	4,21  It has been proposed that the binding of AMP to the AMPK makes it a better substrate whereas the binding of ATP makes it a poor substrate for the upstream kinase.	bind
26907	4	8147	6	13	NULL	NULL	NULL	statement 1	Process		increases					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_4_323_s_133	16051890	4,21  It has been proposed that the binding of AMP to the AMPK makes it a better substrate whereas the binding of ATP makes it a poor substrate for the upstream kinase.	bind
26908	5	8147	6	13	NULL	NULL	NULL	statement 2	Process		decreases					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_4_323_s_133	16051890	4,21  It has been proposed that the binding of AMP to the AMPK makes it a better substrate whereas the binding of ATP makes it a poor substrate for the upstream kinase.	bind
32611	1	8147	7	NULL	NULL	0	NULL	AMP	NULL		bind	NULL				AMPK	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_4_323_s_133	16051890	4,21  It has been proposed that the binding of AMP to the AMPK makes it a better substrate whereas the binding of ATP makes it a poor substrate for the upstream kinase.	bind
32612	2	8147	7	10	NULL	0	NULL	statement 1	NULL		 substrate for	NULL	better			upstream kinase	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_4_323_s_133	16051890	4,21  It has been proposed that the binding of AMP to the AMPK makes it a better substrate whereas the binding of ATP makes it a poor substrate for the upstream kinase.	bind
32613	3	8147	7	NULL	NULL	0	NULL	ATP	NULL		bind	NULL				AMPK	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_4_323_s_133	16051890	4,21  It has been proposed that the binding of AMP to the AMPK makes it a better substrate whereas the binding of ATP makes it a poor substrate for the upstream kinase.	bind
32614	4	8147	7	10	NULL	0	NULL	statement 3	NULL		substrate for	NULL	poor			upstream kinase	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_4_323_s_133	16051890	4,21  It has been proposed that the binding of AMP to the AMPK makes it a better substrate whereas the binding of ATP makes it a poor substrate for the upstream kinase.	bind
26683	1	8148	6	13	NULL	NULL	NULL	lithium	Chemical		inhibits					GSK-3beta	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_7_863_s_7	16614310	4,5  GSK-3beta can be inhibited by lithium and SB415286, which interfere with the binding of ATP to GSK-3 6 rather than acting directly on GSK-3 phosphorylation.	bind
26684	2	8148	6	13	NULL	NULL	NULL	SB415286	Chemical		inhibits					GSK-3beta	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_7_863_s_7	16614310	4,5  GSK-3beta can be inhibited by lithium and SB415286, which interfere with the binding of ATP to GSK-3 6 rather than acting directly on GSK-3 phosphorylation.	bind
26685	3	8148	6	13	NULL	NULL	NULL	ATP	Chemical		bind					GSK-3	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_7_863_s_7	16614310	4,5  GSK-3beta can be inhibited by lithium and SB415286, which interfere with the binding of ATP to GSK-3 6 rather than acting directly on GSK-3 phosphorylation.	bind
26709	4	8148	6	13	NULL	NULL	NULL	lithium	Chemical		interferes with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_7_863_s_7	16614310	4,5  GSK-3beta can be inhibited by lithium and SB415286, which interfere with the binding of ATP to GSK-3 6 rather than acting directly on GSK-3 phosphorylation.	bind
26710	5	8148	6	13	NULL	NULL	NULL	SB415286	Chemical		interferes with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_7_863_s_7	16614310	4,5  GSK-3beta can be inhibited by lithium and SB415286, which interfere with the binding of ATP to GSK-3 6 rather than acting directly on GSK-3 phosphorylation.	bind
55942	6	8148	6	13	NULL	NULL	NULL	GSK-3	GP		undergoes					phosphorylation	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_7_863_s_7	16614310	4,5  GSK-3beta can be inhibited by lithium and SB415286, which interfere with the binding of ATP to GSK-3 6 rather than acting directly on GSK-3 phosphorylation.	bind
55943	7	8148	6	13	NULL	NULL	NULL	lithium	Chemical		does not act on		directly			statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_7_863_s_7	16614310	4,5  GSK-3beta can be inhibited by lithium and SB415286, which interfere with the binding of ATP to GSK-3 6 rather than acting directly on GSK-3 phosphorylation.	bind
55944	8	8148	6	13	NULL	NULL	NULL	SB415286	Chemical		does not act on		directly			statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_7_863_s_7	16614310	4,5  GSK-3beta can be inhibited by lithium and SB415286, which interfere with the binding of ATP to GSK-3 6 rather than acting directly on GSK-3 phosphorylation.	bind
32615	1	8148	7	NULL	NULL	0	NULL	ATP	NULL		bind	NULL				GSK-3	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_7_863_s_7	16614310	4,5  GSK-3beta can be inhibited by lithium and SB415286, which interfere with the binding of ATP to GSK-3 6 rather than acting directly on GSK-3 phosphorylation.	bind
32616	2	8148	7	NULL	NULL	0	NULL	lithium	NULL		inhibits	NULL				GSK-3beta	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_7_863_s_7	16614310	4,5  GSK-3beta can be inhibited by lithium and SB415286, which interfere with the binding of ATP to GSK-3 6 rather than acting directly on GSK-3 phosphorylation.	bind
32617	3	8148	7	NULL	NULL	0	NULL	SB415286	NULL		inhibits	NULL				GSK-3beta	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_7_863_s_7	16614310	4,5  GSK-3beta can be inhibited by lithium and SB415286, which interfere with the binding of ATP to GSK-3 6 rather than acting directly on GSK-3 phosphorylation.	bind
32618	4	8148	7	10	NULL	0	NULL	lithium			interferes with					statement 1					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_7_863_s_7	16614310	4,5  GSK-3beta can be inhibited by lithium and SB415286, which interfere with the binding of ATP to GSK-3 6 rather than acting directly on GSK-3 phosphorylation.	bind
32619	5	8148	7	10	NULL	0	NULL	SB415286			interferes with					statement 1					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_7_863_s_7	16614310	4,5  GSK-3beta can be inhibited by lithium and SB415286, which interfere with the binding of ATP to GSK-3 6 rather than acting directly on GSK-3 phosphorylation.	bind
32620	6	8148	7	NULL	NULL	0	NULL	GSK-3	NULL		undergoes	NULL				phosphorylation	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_7_863_s_7	16614310	4,5  GSK-3beta can be inhibited by lithium and SB415286, which interfere with the binding of ATP to GSK-3 6 rather than acting directly on GSK-3 phosphorylation.	bind
32621	7	8148	7	10	NULL	0	NULL	lithium			does not act on		directly			statement 6					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_7_863_s_7	16614310	4,5  GSK-3beta can be inhibited by lithium and SB415286, which interfere with the binding of ATP to GSK-3 6 rather than acting directly on GSK-3 phosphorylation.	bind
32622	8	8148	7	10	NULL	0	NULL	SB415286			does not act on		directly			statement 6					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_7_863_s_7	16614310	4,5  GSK-3beta can be inhibited by lithium and SB415286, which interfere with the binding of ATP to GSK-3 6 rather than acting directly on GSK-3 phosphorylation.	bind
26909	1	8149	6	13	NULL	NULL	NULL	TFPI-alpha	GP		lacks			K3 domain		proteinase inhibitory activity	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_23_3567_s_21	15557366	4,5  The Kunitz-1 and 2 domains are responsible for TFPI binding and inhibition of TF-FVIIa complex and FXa, respectively, whereas the K3 domain in TFPI-alpha appears to lack proteinase inhibitory activity, and its physiological function is not known.	bind
26912	2	8149	6	13	NULL	NULL	NULL	TFPI	GP		is responsible for			Kunitz-1 domain		TFPI	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_23_3567_s_21	15557366	4,5  The Kunitz-1 and 2 domains are responsible for TFPI binding and inhibition of TF-FVIIa complex and FXa, respectively, whereas the K3 domain in TFPI-alpha appears to lack proteinase inhibitory activity, and its physiological function is not known.	bind
26913	3	8149	6	13	NULL	NULL	NULL	TFPI	GP		plays a role in			Kunitz-1 domain		TFPI	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_23_3567_s_21	15557366	4,5  The Kunitz-1 and 2 domains are responsible for TFPI binding and inhibition of TF-FVIIa complex and FXa, respectively, whereas the K3 domain in TFPI-alpha appears to lack proteinase inhibitory activity, and its physiological function is not known.	bind
26914	4	8149	6	13	NULL	NULL	NULL	TFPI	GP		inhibits			Kunitz-2 domain		TF-FVIIa complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_23_3567_s_21	15557366	4,5  The Kunitz-1 and 2 domains are responsible for TFPI binding and inhibition of TF-FVIIa complex and FXa, respectively, whereas the K3 domain in TFPI-alpha appears to lack proteinase inhibitory activity, and its physiological function is not known.	bind
26915	5	8149	6	13	NULL	NULL	NULL	TFPI	GP		inhibits			Kunitz-2 domain		FXa	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_110_23_3567_s_21	15557366	4,5  The Kunitz-1 and 2 domains are responsible for TFPI binding and inhibition of TF-FVIIa complex and FXa, respectively, whereas the K3 domain in TFPI-alpha appears to lack proteinase inhibitory activity, and its physiological function is not known.	bind
32623	1	8149	7	NULL	NULL	0	NULL		NULL		is responsible for	NULL		Kunitz-1 domain		TFPI	NULL	binding of			NULL		0	NULL	NULL	NULL	gw70_circulation_110_23_3567_s_21	15557366	4,5  The Kunitz-1 and 2 domains are responsible for TFPI binding and inhibition of TF-FVIIa complex and FXa, respectively, whereas the K3 domain in TFPI-alpha appears to lack proteinase inhibitory activity, and its physiological function is not known.	bind
32624	2	8149	7	NULL	NULL	0	NULL		NULL		is responsible for	NULL		Kunitz-2 domain		TFPI	NULL	binding of			NULL		0	NULL	NULL	NULL	gw70_circulation_110_23_3567_s_21	15557366	4,5  The Kunitz-1 and 2 domains are responsible for TFPI binding and inhibition of TF-FVIIa complex and FXa, respectively, whereas the K3 domain in TFPI-alpha appears to lack proteinase inhibitory activity, and its physiological function is not known.	bind
32625	3	8149	7	NULL	NULL	0	NULL		NULL		inhibits	NULL		Kunitz-1 domain		TF-FVIIa complex	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_110_23_3567_s_21	15557366	4,5  The Kunitz-1 and 2 domains are responsible for TFPI binding and inhibition of TF-FVIIa complex and FXa, respectively, whereas the K3 domain in TFPI-alpha appears to lack proteinase inhibitory activity, and its physiological function is not known.	bind
32626	4	8149	7	NULL	NULL	0	NULL		NULL		inhibits	NULL		Kunitz-2 domain		FXa	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_110_23_3567_s_21	15557366	4,5  The Kunitz-1 and 2 domains are responsible for TFPI binding and inhibition of TF-FVIIa complex and FXa, respectively, whereas the K3 domain in TFPI-alpha appears to lack proteinase inhibitory activity, and its physiological function is not known.	bind
32627	5	8149	7	NULL	NULL	0	NULL	TFPI-alpha	NULL		lack 	NULL		K3 domain		proteinase inhibitory activity	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_110_23_3567_s_21	15557366	4,5  The Kunitz-1 and 2 domains are responsible for TFPI binding and inhibition of TF-FVIIa complex and FXa, respectively, whereas the K3 domain in TFPI-alpha appears to lack proteinase inhibitory activity, and its physiological function is not known.	bind
26711	1	8150	6	13	NULL	NULL	NULL	c-Src	GP		bind					Cx43CT	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_2_215_s_141	14699011	4,5  To test this hypothesis, we used RMS to evaluate whether c-Src binding to Cx43CT interferes with binding of ZO-1 ( Figure 6).	bind
26712	2	8150	6	13	NULL	NULL	NULL	statement 1	Process		interfere with		may			ZO-1	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_2_215_s_141	14699011	4,5  To test this hypothesis, we used RMS to evaluate whether c-Src binding to Cx43CT interferes with binding of ZO-1 ( Figure 6).	bind
32630	1	8150	7	NULL	NULL	0	NULL	 c-Src	NULL		bind	NULL				Cx43CT	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_2_215_s_141	14699011	4,5  To test this hypothesis, we used RMS to evaluate whether c-Src binding to Cx43CT interferes with binding of ZO-1 ( Figure 6).	bind
32631	2	8150	7	10	NULL	0	NULL	statement 1			interfere with		may			ZO-1		binding of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_2_215_s_141	14699011	4,5  To test this hypothesis, we used RMS to evaluate whether c-Src binding to Cx43CT interferes with binding of ZO-1 ( Figure 6).	bind
26714	1	8152	6	13	NULL	NULL	NULL	GPCR	GP		transactivate					EGFR	GP				NULL	cardiomyocytes	NULL	NULL	NULL	NULL	gw70_circulationres_94_1_68_s_18	14656925	4,8 - 12      These GPCRs transactivate the EGF receptor (EGFR) in cardiomyocytes via a shared pathway, whereby ADAM 12 sheds membrane-anchored HB-EGF, which then binds to the EGFR either directly or via an interaction with the proteoglycan matrix or cell membrane molecules (such as CD44) to signal growth.	bind
26715	2	8152	6	13	NULL	NULL	NULL	EGFR	GP		is					EGF receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_1_68_s_18	14656925	4,8 - 12      These GPCRs transactivate the EGF receptor (EGFR) in cardiomyocytes via a shared pathway, whereby ADAM 12 sheds membrane-anchored HB-EGF, which then binds to the EGFR either directly or via an interaction with the proteoglycan matrix or cell membrane molecules (such as CD44) to signal growth.	bind
26717	3	8152	6	13	NULL	NULL	NULL	ADAM	GP		sheds					HB-EGF	GP	membrane-anchored			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_1_68_s_18	14656925	4,8 - 12      These GPCRs transactivate the EGF receptor (EGFR) in cardiomyocytes via a shared pathway, whereby ADAM 12 sheds membrane-anchored HB-EGF, which then binds to the EGFR either directly or via an interaction with the proteoglycan matrix or cell membrane molecules (such as CD44) to signal growth.	bind
26719	4	8152	6	13	NULL	NULL	NULL	HB-EGF	GP		bind		directly			EGFR	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_1_68_s_18	14656925	4,8 - 12      These GPCRs transactivate the EGF receptor (EGFR) in cardiomyocytes via a shared pathway, whereby ADAM 12 sheds membrane-anchored HB-EGF, which then binds to the EGFR either directly or via an interaction with the proteoglycan matrix or cell membrane molecules (such as CD44) to signal growth.	bind
26720	5	8152	6	13	NULL	NULL	NULL	HB-EGF	GP		interacts with					proteoglycan matrix 	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_1_68_s_18	14656925	4,8 - 12      These GPCRs transactivate the EGF receptor (EGFR) in cardiomyocytes via a shared pathway, whereby ADAM 12 sheds membrane-anchored HB-EGF, which then binds to the EGFR either directly or via an interaction with the proteoglycan matrix or cell membrane molecules (such as CD44) to signal growth.	bind
26724	6	8152	6	13	NULL	NULL	NULL	HB-EGF	GP		bind					CD44	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_1_68_s_18	14656925	4,8 - 12      These GPCRs transactivate the EGF receptor (EGFR) in cardiomyocytes via a shared pathway, whereby ADAM 12 sheds membrane-anchored HB-EGF, which then binds to the EGFR either directly or via an interaction with the proteoglycan matrix or cell membrane molecules (such as CD44) to signal growth.	bind
26726	7	8152	6	13	NULL	NULL	NULL	CD44	GP		is a type of					cell membrane molecule	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_1_68_s_18	14656925	4,8 - 12      These GPCRs transactivate the EGF receptor (EGFR) in cardiomyocytes via a shared pathway, whereby ADAM 12 sheds membrane-anchored HB-EGF, which then binds to the EGFR either directly or via an interaction with the proteoglycan matrix or cell membrane molecules (such as CD44) to signal growth.	bind
32634	1	8152	7	NULL	NULL	0	NULL	GPCRs 	NULL		transactivate	NULL				EGFR	NULL				NULL	 cardiomyocytes 	0	NULL	NULL	NULL	gw70_circulationres_94_1_68_s_18	14656925	4,8 - 12      These GPCRs transactivate the EGF receptor (EGFR) in cardiomyocytes via a shared pathway, whereby ADAM 12 sheds membrane-anchored HB-EGF, which then binds to the EGFR either directly or via an interaction with the proteoglycan matrix or cell membrane molecules (such as CD44) to signal growth.	bind
32635	2	8152	7	10	NULL	0	NULL	ADAM 12	NULL		sheds	NULL				HB-EGF	NULL	membrane-anchored			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_1_68_s_18	14656925	4,8 - 12      These GPCRs transactivate the EGF receptor (EGFR) in cardiomyocytes via a shared pathway, whereby ADAM 12 sheds membrane-anchored HB-EGF, which then binds to the EGFR either directly or via an interaction with the proteoglycan matrix or cell membrane molecules (such as CD44) to signal growth.	bind
32636	3	8152	7	NULL	NULL	0	NULL	statement 1	NULL		via	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_1_68_s_18	14656925	4,8 - 12      These GPCRs transactivate the EGF receptor (EGFR) in cardiomyocytes via a shared pathway, whereby ADAM 12 sheds membrane-anchored HB-EGF, which then binds to the EGFR either directly or via an interaction with the proteoglycan matrix or cell membrane molecules (such as CD44) to signal growth.	bind
32637	4	8152	7	NULL	NULL	0	NULL	HB-EGF	NULL		bind	NULL	directly			EGFR	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_1_68_s_18	14656925	4,8 - 12      These GPCRs transactivate the EGF receptor (EGFR) in cardiomyocytes via a shared pathway, whereby ADAM 12 sheds membrane-anchored HB-EGF, which then binds to the EGFR either directly or via an interaction with the proteoglycan matrix or cell membrane molecules (such as CD44) to signal growth.	bind
32640	5	8152	7	NULL	NULL	0	NULL	HB-EGF	NULL		interacts with	NULL				proteoglycan matrix	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_1_68_s_18	14656925	4,8 - 12      These GPCRs transactivate the EGF receptor (EGFR) in cardiomyocytes via a shared pathway, whereby ADAM 12 sheds membrane-anchored HB-EGF, which then binds to the EGFR either directly or via an interaction with the proteoglycan matrix or cell membrane molecules (such as CD44) to signal growth.	bind
32644	6	8152	7	NULL	NULL	0	NULL	HB-EGF	NULL		bind	NULL				CD44	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_1_68_s_18	14656925	4,8 - 12      These GPCRs transactivate the EGF receptor (EGFR) in cardiomyocytes via a shared pathway, whereby ADAM 12 sheds membrane-anchored HB-EGF, which then binds to the EGFR either directly or via an interaction with the proteoglycan matrix or cell membrane molecules (such as CD44) to signal growth.	bind
32645	7	8152	7	NULL	NULL	0	NULL	EGFR	NULL		is	NULL				EGF receptor	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_1_68_s_18	14656925	4,8 - 12      These GPCRs transactivate the EGF receptor (EGFR) in cardiomyocytes via a shared pathway, whereby ADAM 12 sheds membrane-anchored HB-EGF, which then binds to the EGFR either directly or via an interaction with the proteoglycan matrix or cell membrane molecules (such as CD44) to signal growth.	bind
32648	8	8152	7	NULL	NULL	0	NULL	CD44	NULL		is a type of	NULL				cell membrane molecule	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_1_68_s_18	14656925	4,8 - 12      These GPCRs transactivate the EGF receptor (EGFR) in cardiomyocytes via a shared pathway, whereby ADAM 12 sheds membrane-anchored HB-EGF, which then binds to the EGFR either directly or via an interaction with the proteoglycan matrix or cell membrane molecules (such as CD44) to signal growth.	bind
32662	9	8152	7	NULL	NULL	0	NULL	statement 4	NULL		signal	NULL				growth	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_1_68_s_18	14656925	4,8 - 12      These GPCRs transactivate the EGF receptor (EGFR) in cardiomyocytes via a shared pathway, whereby ADAM 12 sheds membrane-anchored HB-EGF, which then binds to the EGFR either directly or via an interaction with the proteoglycan matrix or cell membrane molecules (such as CD44) to signal growth.	bind
32663	10	8152	7	NULL	NULL	0	NULL	statement 5	NULL		signal	NULL				growth	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_1_68_s_18	14656925	4,8 - 12      These GPCRs transactivate the EGF receptor (EGFR) in cardiomyocytes via a shared pathway, whereby ADAM 12 sheds membrane-anchored HB-EGF, which then binds to the EGFR either directly or via an interaction with the proteoglycan matrix or cell membrane molecules (such as CD44) to signal growth.	bind
32664	11	8152	7	NULL	NULL	0	NULL	statement 6	NULL		signal	NULL				growth	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_1_68_s_18	14656925	4,8 - 12      These GPCRs transactivate the EGF receptor (EGFR) in cardiomyocytes via a shared pathway, whereby ADAM 12 sheds membrane-anchored HB-EGF, which then binds to the EGFR either directly or via an interaction with the proteoglycan matrix or cell membrane molecules (such as CD44) to signal growth.	bind
26727	1	8153	6	13	NULL	NULL	NULL	FasL	GP		bind					Fas	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_1_153_s_14	11141488	4- 7  Binding of FasL to Fas results in apoptosis of susceptible cells.	bind
26728	2	8153	6	13	NULL	NULL	NULL	statement 1	Process		results in					susceptible cell	Cell	apoptosis of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_158_1_153_s_14	11141488	4- 7  Binding of FasL to Fas results in apoptosis of susceptible cells.	bind
32665	1	8153	7	NULL	NULL	0	NULL	 FasL 	NULL		bind	NULL				Fas	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_1_153_s_14	11141488	4- 7  Binding of FasL to Fas results in apoptosis of susceptible cells.	bind
32666	2	8153	7	NULL	NULL	0	NULL	statement 1	NULL		results in	NULL				susceptible cells	NULL	apoptosis of 			NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_1_153_s_14	11141488	4- 7  Binding of FasL to Fas results in apoptosis of susceptible cells.	bind
26730	1	8154	6	13	NULL	NULL	NULL	T cell antigen	Chemical		bind					B cells	Cell	mature			NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_23_0_23_s_1462	15771565	4-1BB T cell  antigen binds to mature B cells and macrophages, and costimulates anti- -primed splenic  B cells.	bind
26736	2	8154	6	13	NULL	NULL	NULL	T cell antigen	Chemical		bind					macrophages	Cell				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_23_0_23_s_1462	15771565	4-1BB T cell  antigen binds to mature B cells and macrophages, and costimulates anti- -primed splenic  B cells.	bind
26737	3	8154	6	13	NULL	NULL	NULL	T cell antigen	Chemical		costimulates					B cells	Cell	anti--primed;;splenic			NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_23_0_23_s_1462	15771565	4-1BB T cell  antigen binds to mature B cells and macrophages, and costimulates anti- -primed splenic  B cells.	bind
32667	1	8154	7	10	NULL	0	NULL	T cell antigen			binds to					B cells		mature			NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_23_0_23_s_1462	15771565	4-1BB T cell  antigen binds to mature B cells and macrophages, and costimulates anti- -primed splenic  B cells.	bind
32668	2	8154	7	10	NULL	0	NULL	T cell antigen			binds to					macrophages					NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_23_0_23_s_1462	15771565	4-1BB T cell  antigen binds to mature B cells and macrophages, and costimulates anti- -primed splenic  B cells.	bind
32669	3	8154	7	10	NULL	0	NULL	T cell antigen			costimulates					B cells		anti--primed;;splenic			NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_23_0_23_s_1462	15771565	4-1BB T cell  antigen binds to mature B cells and macrophages, and costimulates anti- -primed splenic  B cells.	bind
32670	1	8155	7	13	NULL	NULL	NULL	T-cell antigen	Chemical		binds to					B cells	Cell	mature			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_71_1_196_s_368	12496166	4-1BB T-cell antigen binds to mature B cells and macrophage, and costimulates anti-mu-primed splenic B cells.	bind
32671	2	8155	7	13	NULL	NULL	NULL	T-cell antigen	Chemical		binds to					macrophages	Cell				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_71_1_196_s_368	12496166	4-1BB T-cell antigen binds to mature B cells and macrophage, and costimulates anti-mu-primed splenic B cells.	bind
32672	3	8155	7	13	NULL	NULL	NULL	T-cell antigen	Chemical		costimulates					B cells	Cell	anti-mu-primed;;splenic			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_71_1_196_s_368	12496166	4-1BB T-cell antigen binds to mature B cells and macrophage, and costimulates anti-mu-primed splenic B cells.	bind
26738	1	8156	6	13	NULL	NULL	NULL	4-DAMP mustard	Chemical		bind					mACh receptors	GP				NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_314_2_891_s_20	15857948	4-Diphenylacetoxy- N-(2-chloroethyl)piperidine (4-DAMP mustard) is known to bind to mACh receptors (Thomas et al., 1992 ; Eglen et al., 1994 ; Ehlert and Griffin, 1998 ; Sawyer and Ehlert, 1999 ; Ragheb et al., 2001 ; Umland et al., 2001 ) with moderate selectivity for M3-mACh receptors.	bind
26739	2	8156	6	13	NULL	NULL	NULL	4-DAMP mustard	Chemical		is					4-Diphenylacetoxy- N-(2-chloroethyl)piperidine	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_314_2_891_s_20	15857948	4-Diphenylacetoxy- N-(2-chloroethyl)piperidine (4-DAMP mustard) is known to bind to mACh receptors (Thomas et al., 1992 ; Eglen et al., 1994 ; Ehlert and Griffin, 1998 ; Sawyer and Ehlert, 1999 ; Ragheb et al., 2001 ; Umland et al., 2001 ) with moderate selectivity for M3-mACh receptors.	bind
32673	1	8156	7	NULL	NULL	0	NULL	4-DAMP mustard	NULL		bind	NULL				mACh receptors	NULL				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_314_2_891_s_20	15857948	4-Diphenylacetoxy- N-(2-chloroethyl)piperidine (4-DAMP mustard) is known to bind to mACh receptors (Thomas et al., 1992 ; Eglen et al., 1994 ; Ehlert and Griffin, 1998 ; Sawyer and Ehlert, 1999 ; Ragheb et al., 2001 ; Umland et al., 2001 ) with moderate selectivity for M3-mACh receptors.	bind
32675	3	8156	7	NULL	NULL	0	NULL	4-DAMP	NULL		is	NULL				4-Diphenylacetoxy- N-(2-chloroethyl)piperidine 	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_314_2_891_s_20	15857948	4-Diphenylacetoxy- N-(2-chloroethyl)piperidine (4-DAMP mustard) is known to bind to mACh receptors (Thomas et al., 1992 ; Eglen et al., 1994 ; Ehlert and Griffin, 1998 ; Sawyer and Ehlert, 1999 ; Ragheb et al., 2001 ; Umland et al., 2001 ) with moderate selectivity for M3-mACh receptors.	bind
32676	4	8156	7	10	NULL	0	NULL	4-DAMP mustard	NULL		selectivity for	NULL	moderate			M3-mACh receptors	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_314_2_891_s_20	15857948	4-Diphenylacetoxy- N-(2-chloroethyl)piperidine (4-DAMP mustard) is known to bind to mACh receptors (Thomas et al., 1992 ; Eglen et al., 1994 ; Ehlert and Griffin, 1998 ; Sawyer and Ehlert, 1999 ; Ragheb et al., 2001 ; Umland et al., 2001 ) with moderate selectivity for M3-mACh receptors.	bind
26740	1	8157	6	13	NULL	NULL	NULL	4-Hydroxybutyrate dehydrogenase	GP		requires					NAD(H)	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_65_9_3901_s_141	10473393	4-Hydroxybutyrate dehydrogenase requires NAD(H) as a cofactor, but the highly conserved NAD(H) binding fingerprint pattern G-X-G-X-X-G ( 15) was not present in the amino acid sequence.	bind
26741	2	8157	6	13	NULL	NULL	NULL	NAD(H)	Chemical		acts as a 					cofactor	Chemical				NULL	statement 1	NULL	NULL	NULL	NULL	gw60_applenvironmicrob_65_9_3901_s_141	10473393	4-Hydroxybutyrate dehydrogenase requires NAD(H) as a cofactor, but the highly conserved NAD(H) binding fingerprint pattern G-X-G-X-X-G ( 15) was not present in the amino acid sequence.	bind
26742	3	8157	6	13	NULL	NULL	NULL				is the fingerprint pattern for		highly conserved	G-X-G-X-X-G		NAD(H)	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_65_9_3901_s_141	10473393	4-Hydroxybutyrate dehydrogenase requires NAD(H) as a cofactor, but the highly conserved NAD(H) binding fingerprint pattern G-X-G-X-X-G ( 15) was not present in the amino acid sequence.	bind
32677	1	8157	7	NULL	NULL	0	NULL	4-Hydroxybutyrate dehydrogenase	NULL		requires	NULL				NAD(H) cofactor	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_9_3901_s_141	10473393	4-Hydroxybutyrate dehydrogenase requires NAD(H) as a cofactor, but the highly conserved NAD(H) binding fingerprint pattern G-X-G-X-X-G ( 15) was not present in the amino acid sequence.	bind
32678	2	8157	7	10	NULL	0	NULL		NULL		is not present in	NULL		G-X-G-X-X-G		4-Hydroxybutyrate dehydrogenase	NULL				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_65_9_3901_s_141	10473393	4-Hydroxybutyrate dehydrogenase requires NAD(H) as a cofactor, but the highly conserved NAD(H) binding fingerprint pattern G-X-G-X-X-G ( 15) was not present in the amino acid sequence.	bind
46579	3	8157	7	10	NULL	0	NULL	G-X-G-X-X-G	NULL		is the fingerprint pattern for	NULL	highly conserved			NAD(H)	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_65_9_3901_s_141	10473393	4-Hydroxybutyrate dehydrogenase requires NAD(H) as a cofactor, but the highly conserved NAD(H) binding fingerprint pattern G-X-G-X-X-G ( 15) was not present in the amino acid sequence.	bind
26743	1	8158	6	13	NULL	NULL	NULL	mTAb1	GP		bind					mTOR	GP				NULL	MER-Akt cells	NULL	NULL	NULL	NULL	gw60_pnas_95_13_7772_s_163	9636226	4-Hydroxytamoxifen rapidly decreased mTAb1 binding to mTOR in the MER-Akt cells, but not in the parental NIH 3T3 cells (Fig.  5 A).	bind
26744	2	8158	6	13	NULL	NULL	NULL	mTAb1	GP		bind					mTOR	GP				NULL	parental NIH 3T3 cells	NULL	NULL	NULL	NULL	gw60_pnas_95_13_7772_s_163	9636226	4-Hydroxytamoxifen rapidly decreased mTAb1 binding to mTOR in the MER-Akt cells, but not in the parental NIH 3T3 cells (Fig.  5 A).	bind
26745	3	8158	6	13	NULL	NULL	NULL	Hydroxytamoxifen	Chemical		decreases		rapidly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_13_7772_s_163	9636226	4-Hydroxytamoxifen rapidly decreased mTAb1 binding to mTOR in the MER-Akt cells, but not in the parental NIH 3T3 cells (Fig.  5 A).	bind
26746	4	8158	6	13	NULL	NULL	NULL	Hydroxytamoxifen	Chemical		does not decrease					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_13_7772_s_163	9636226	4-Hydroxytamoxifen rapidly decreased mTAb1 binding to mTOR in the MER-Akt cells, but not in the parental NIH 3T3 cells (Fig.  5 A).	bind
32679	1	8158	7	NULL	NULL	0	NULL	mTAb1	NULL		bind	NULL				mTOR	NULL				NULL	MER-Akt cells	0	NULL	NULL	NULL	gw60_pnas_95_13_7772_s_163	9636226	4-Hydroxytamoxifen rapidly decreased mTAb1 binding to mTOR in the MER-Akt cells, but not in the parental NIH 3T3 cells (Fig.  5 A).	bind
32680	2	8158	7	NULL	NULL	0	NULL	4-Hydroxytamoxifen	NULL		decrease	NULL	rapidly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_13_7772_s_163	9636226	4-Hydroxytamoxifen rapidly decreased mTAb1 binding to mTOR in the MER-Akt cells, but not in the parental NIH 3T3 cells (Fig.  5 A).	bind
32681	3	8158	7	NULL	NULL	0	NULL	 mTAb1	NULL		bind	NULL				mTOR	NULL				NULL	 parental NIH 3T3 cells 	0	NULL	NULL	NULL	gw60_pnas_95_13_7772_s_163	9636226	4-Hydroxytamoxifen rapidly decreased mTAb1 binding to mTOR in the MER-Akt cells, but not in the parental NIH 3T3 cells (Fig.  5 A).	bind
32682	4	8158	7	NULL	NULL	0	NULL	4-Hydroxytamoxifen	NULL		does not decrease	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_13_7772_s_163	9636226	4-Hydroxytamoxifen rapidly decreased mTAb1 binding to mTOR in the MER-Akt cells, but not in the parental NIH 3T3 cells (Fig.  5 A).	bind
26747	1	8159	6	13	NULL	NULL	NULL	4-oxo-RA	Chemical		bind					atRA binding proteins	GP	cellular			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_10_6908_s_218	10702251	4-oxo-RA can also bind to cellular atRA binding proteins ( 40).	bind
32683	1	8159	7	10	NULL	0	NULL	4-oxo-RA	NULL		bind	NULL				atRA binding protein	NULL	cellular			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_10_6908_s_218	10702251	4-oxo-RA can also bind to cellular atRA binding proteins ( 40).	bind
26748	1	8160	6	13	NULL	NULL	NULL	E2	Chemical		bind					ER	GP				NULL	MCF-7 cells	NULL	NULL	NULL	NULL	abs-batch0600-0619_j-toxicol-environ-health-a_65_5-6_11936222_s_8	11936222	4-t-Octylphenol and  4-nonylphenol inhibited the binding of E2 to the ER of MCF-7 cells in  a competitive ER binding assay.	bind
26749	2	8160	6	13	NULL	NULL	NULL	4-t-Octylphenol	Chemical		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_j-toxicol-environ-health-a_65_5-6_11936222_s_8	11936222	4-t-Octylphenol and  4-nonylphenol inhibited the binding of E2 to the ER of MCF-7 cells in  a competitive ER binding assay.	bind
26750	3	8160	6	13	NULL	NULL	NULL	4-nonylphenol	Chemical		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_j-toxicol-environ-health-a_65_5-6_11936222_s_8	11936222	4-t-Octylphenol and  4-nonylphenol inhibited the binding of E2 to the ER of MCF-7 cells in  a competitive ER binding assay.	bind
32684	1	8160	7	NULL	NULL	0	NULL	 E2 	NULL		bind	NULL				ER	NULL				NULL	MCF-7 cells	0	NULL	NULL	NULL	abs-batch0600-0619_j-toxicol-environ-health-a_65_5-6_11936222_s_8	11936222	4-t-Octylphenol and  4-nonylphenol inhibited the binding of E2 to the ER of MCF-7 cells in  a competitive ER binding assay.	bind
32685	2	8160	7	NULL	NULL	0	NULL	4-t-Octylphenol	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0600-0619_j-toxicol-environ-health-a_65_5-6_11936222_s_8	11936222	4-t-Octylphenol and  4-nonylphenol inhibited the binding of E2 to the ER of MCF-7 cells in  a competitive ER binding assay.	bind
32686	3	8160	7	NULL	NULL	0	NULL	4-nonylphenol	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0600-0619_j-toxicol-environ-health-a_65_5-6_11936222_s_8	11936222	4-t-Octylphenol and  4-nonylphenol inhibited the binding of E2 to the ER of MCF-7 cells in  a competitive ER binding assay.	bind
26751	1	8161	6	13	NULL	NULL	NULL	r30kDa	GP		bind					GPC-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24540_s_86	10831591	4.1 and r30kDa also bound GPC-3 with a  K( D)kin value on the order of 0.1 muM (Table  I), but no binding could be documented between r30kDa and either GPC-1 or GPC-2	bind
26752	2	8161	6	13	NULL	NULL	NULL	r30kDa	GP		does not bind					GPC-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24540_s_86	10831591	4.1 and r30kDa also bound GPC-3 with a  K( D)kin value on the order of 0.1 muM (Table  I), but no binding could be documented between r30kDa and either GPC-1 or GPC-2	bind
26753	3	8161	6	13	NULL	NULL	NULL	r30kDa	GP		does not bind					GPC-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24540_s_86	10831591	4.1 and r30kDa also bound GPC-3 with a  K( D)kin value on the order of 0.1 muM (Table  I), but no binding could be documented between r30kDa and either GPC-1 or GPC-2	bind
32687	1	8161	7	NULL	NULL	0	NULL	r30kDa	NULL		bind	NULL				GPC-3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24540_s_86	10831591	4.1 and r30kDa also bound GPC-3 with a  K( D)kin value on the order of 0.1 muM (Table  I), but no binding could be documented between r30kDa and either GPC-1 or GPC-2	bind
32688	2	8161	7	NULL	NULL	0	NULL	 r30kDa	NULL		does not bind	NULL				 GPC-1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24540_s_86	10831591	4.1 and r30kDa also bound GPC-3 with a  K( D)kin value on the order of 0.1 muM (Table  I), but no binding could be documented between r30kDa and either GPC-1 or GPC-2	bind
32689	3	8161	7	NULL	NULL	0	NULL	r30kDa	NULL		does not bind	NULL				 GPC-2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24540_s_86	10831591	4.1 and r30kDa also bound GPC-3 with a  K( D)kin value on the order of 0.1 muM (Table  I), but no binding could be documented between r30kDa and either GPC-1 or GPC-2	bind
26754	1	8162	6	13	NULL	NULL	NULL	SAP97	GP		bind					AMPAR	GP		GluR1 subunits		NULL	hippocampal synapses	NULL	NULL	NULL	NULL	gw60_neuron_31_2_191_s_139	11502252	4.1 and SAP97 are the major binding partners for the GluR1 subunits of AMPARs at hippocampal synapses     (Leonard et al., 1998  ; Shen et al., 2000b  ; Valtschanoff et al., 2000  ; Walensky et al., 1999  ) and form sites where AMPARs can anchor.	bind
32690	1	8162	7	NULL	NULL	0	NULL	 SAP97 	NULL		bind	NULL				AMPARs	NULL		GluR1 subunits 		NULL	hippocampal synapses	0	NULL	NULL	NULL	gw60_neuron_31_2_191_s_139	11502252	4.1 and SAP97 are the major binding partners for the GluR1 subunits of AMPARs at hippocampal synapses     (Leonard et al., 1998  ; Shen et al., 2000b  ; Valtschanoff et al., 2000  ; Walensky et al., 1999  ) and form sites where AMPARs can anchor.	bind
26755	1	8163	6	13	NULL	NULL	NULL	p55	GP		bind					GPC	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24540_s_134	10831591	4.1 Modulates p55 Binding to GPC, but p55 Does Not Affect 4.1 Binding to GPC-- To further define the interactions among the three protein components of the ternary complex, 4.1, p55, and GPC, we determined whether p55-GPC and 4.1-GPC binary interactions can be regulated by the third member of the complex, namely, 4.1 and p55, respectively.	bind
26756	2	8163	6	13	NULL	NULL	NULL	4.1	GP		modulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24540_s_134	10831591	4.1 Modulates p55 Binding to GPC, but p55 Does Not Affect 4.1 Binding to GPC-- To further define the interactions among the three protein components of the ternary complex, 4.1, p55, and GPC, we determined whether p55-GPC and 4.1-GPC binary interactions can be regulated by the third member of the complex, namely, 4.1 and p55, respectively.	bind
26757	3	8163	6	13	NULL	NULL	NULL	4.1	GP		bind					GPC	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24540_s_134	10831591	4.1 Modulates p55 Binding to GPC, but p55 Does Not Affect 4.1 Binding to GPC-- To further define the interactions among the three protein components of the ternary complex, 4.1, p55, and GPC, we determined whether p55-GPC and 4.1-GPC binary interactions can be regulated by the third member of the complex, namely, 4.1 and p55, respectively.	bind
26758	4	8163	6	13	NULL	NULL	NULL	p55	GP		does not affect					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24540_s_134	10831591	4.1 Modulates p55 Binding to GPC, but p55 Does Not Affect 4.1 Binding to GPC-- To further define the interactions among the three protein components of the ternary complex, 4.1, p55, and GPC, we determined whether p55-GPC and 4.1-GPC binary interactions can be regulated by the third member of the complex, namely, 4.1 and p55, respectively.	bind
32692	1	8163	7	NULL	NULL	0	NULL	p55	NULL		bind	NULL				GPC	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24540_s_134	10831591	4.1 Modulates p55 Binding to GPC, but p55 Does Not Affect 4.1 Binding to GPC-- To further define the interactions among the three protein components of the ternary complex, 4.1, p55, and GPC, we determined whether p55-GPC and 4.1-GPC binary interactions can be regulated by the third member of the complex, namely, 4.1 and p55, respectively.	bind
32693	2	8163	7	NULL	NULL	0	NULL	4.1	NULL		modulates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24540_s_134	10831591	4.1 Modulates p55 Binding to GPC, but p55 Does Not Affect 4.1 Binding to GPC-- To further define the interactions among the three protein components of the ternary complex, 4.1, p55, and GPC, we determined whether p55-GPC and 4.1-GPC binary interactions can be regulated by the third member of the complex, namely, 4.1 and p55, respectively.	bind
32694	3	8163	7	NULL	NULL	0	NULL	 4.1	NULL		bind	NULL				GPC	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24540_s_134	10831591	4.1 Modulates p55 Binding to GPC, but p55 Does Not Affect 4.1 Binding to GPC-- To further define the interactions among the three protein components of the ternary complex, 4.1, p55, and GPC, we determined whether p55-GPC and 4.1-GPC binary interactions can be regulated by the third member of the complex, namely, 4.1 and p55, respectively.	bind
32695	4	8163	7	NULL	NULL	0	NULL	p55 	NULL		does not affect	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24540_s_134	10831591	4.1 Modulates p55 Binding to GPC, but p55 Does Not Affect 4.1 Binding to GPC-- To further define the interactions among the three protein components of the ternary complex, 4.1, p55, and GPC, we determined whether p55-GPC and 4.1-GPC binary interactions can be regulated by the third member of the complex, namely, 4.1 and p55, respectively.	bind
26759	1	8164	6	13	NULL	NULL	NULL	4.1G	GP		contains			CTD		peptidyl-prolyl bonds	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_1_143_s_247	9531554	4.1G-CTD contains three peptidyl-prolyl bonds that  could potentially participate in FKBP13 binding, including  val-pro at aa 18-19, ser-pro at 32-33, and his-pro at 107-108.	bind
26760	2	8164	6	13	NULL	NULL	NULL	statement 1	GP		participate in		potentially			FKBP13	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_1_143_s_247	9531554	4.1G-CTD contains three peptidyl-prolyl bonds that  could potentially participate in FKBP13 binding, including  val-pro at aa 18-19, ser-pro at 32-33, and his-pro at 107-108.	bind
26761	3	8164	6	13	NULL	NULL	NULL	4.1G	GP		contains			CTD					val-pro at aa 18-19		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_1_143_s_247	9531554	4.1G-CTD contains three peptidyl-prolyl bonds that  could potentially participate in FKBP13 binding, including  val-pro at aa 18-19, ser-pro at 32-33, and his-pro at 107-108.	bind
26762	4	8164	6	13	NULL	NULL	NULL	4.1G	GP		contains			CTD					ser-pro at 32-33		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_1_143_s_247	9531554	4.1G-CTD contains three peptidyl-prolyl bonds that  could potentially participate in FKBP13 binding, including  val-pro at aa 18-19, ser-pro at 32-33, and his-pro at 107-108.	bind
26763	5	8164	6	13	NULL	NULL	NULL	4.1G	GP		contains			CTD					his-pro at 107-108		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_1_143_s_247	9531554	4.1G-CTD contains three peptidyl-prolyl bonds that  could potentially participate in FKBP13 binding, including  val-pro at aa 18-19, ser-pro at 32-33, and his-pro at 107-108.	bind
32696	1	8164	7	10	NULL	0	NULL	4.1G	NULL		contains	NULL		CTD		peptidyl-prolyl bonds	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_1_143_s_247	9531554	4.1G-CTD contains three peptidyl-prolyl bonds that  could potentially participate in FKBP13 binding, including  val-pro at aa 18-19, ser-pro at 32-33, and his-pro at 107-108.	bind
32697	2	8164	7	10	NULL	0	NULL	4.1G	NULL		participate in	NULL	potentially	CTD		FKBP13	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_1_143_s_247	9531554	4.1G-CTD contains three peptidyl-prolyl bonds that  could potentially participate in FKBP13 binding, including  val-pro at aa 18-19, ser-pro at 32-33, and his-pro at 107-108.	bind
46581	3	8164	7	10	NULL	0	NULL	4.1G	NULL		contains	NULL		CTD			NULL		val-pro at aa 18-19		NULL		0	NULL	NULL	NULL	gw60_cellbiol_141_1_143_s_247	9531554	4.1G-CTD contains three peptidyl-prolyl bonds that  could potentially participate in FKBP13 binding, including  val-pro at aa 18-19, ser-pro at 32-33, and his-pro at 107-108.	bind
46582	4	8164	7	10	NULL	0	NULL	4.1G	NULL		contains	NULL		CTD			NULL		ser-pro at 32-33		NULL		0	NULL	NULL	NULL	gw60_cellbiol_141_1_143_s_247	9531554	4.1G-CTD contains three peptidyl-prolyl bonds that  could potentially participate in FKBP13 binding, including  val-pro at aa 18-19, ser-pro at 32-33, and his-pro at 107-108.	bind
46583	5	8164	7	10	NULL	0	NULL	4.1G	NULL		contains	NULL		CTD			NULL		his-pro at 107-108		NULL		0	NULL	NULL	NULL	gw60_cellbiol_141_1_143_s_247	9531554	4.1G-CTD contains three peptidyl-prolyl bonds that  could potentially participate in FKBP13 binding, including  val-pro at aa 18-19, ser-pro at 32-33, and his-pro at 107-108.	bind
26764	1	8165	6	13	NULL	NULL	NULL	NF1	GP		bind					MMTV	GP			promoter	NULL	nucleosomes	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3448_s_375	11504883	40       Eisfeld,K., Candau,R., Truss,M. and Beato,M. (1997) Binding of NF1 to the MMTV promoter in nucleosomes: influence of rotational phasing, translational positioning and histone H1.	bind
32700	1	8165	7	NULL	NULL	0	NULL	NF1	NULL		bind	NULL				MMTV	NULL			promoter	NULL	nucleosomes	0	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3448_s_375	11504883	40       Eisfeld,K., Candau,R., Truss,M. and Beato,M. (1997) Binding of NF1 to the MMTV promoter in nucleosomes: influence of rotational phasing, translational positioning and histone H1.	bind
26949	1	8166	6	13	NULL	NULL	NULL	Sp1	GP		bind					dihydrofolate reductase	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_783_s_367	11160902	40       Gee,J.E., Blume,S., Snyder,R.C., Ray,R. and Miller,D.M. (1992) Triplex formation prevents Sp1 binding to the dihydrofolate reductase promoter.	bind
26950	2	8166	6	13	NULL	NULL	NULL	triplex formation	GP		prevents					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_783_s_367	11160902	40       Gee,J.E., Blume,S., Snyder,R.C., Ray,R. and Miller,D.M. (1992) Triplex formation prevents Sp1 binding to the dihydrofolate reductase promoter.	bind
32701	1	8166	7	NULL	NULL	0	NULL	 Sp1	NULL		bind	NULL				dihydrofolate reductase	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_783_s_367	11160902	40       Gee,J.E., Blume,S., Snyder,R.C., Ray,R. and Miller,D.M. (1992) Triplex formation prevents Sp1 binding to the dihydrofolate reductase promoter.	bind
32702	2	8166	7	NULL	NULL	0	NULL	Triplex formation 	NULL		prevents	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_783_s_367	11160902	40       Gee,J.E., Blume,S., Snyder,R.C., Ray,R. and Miller,D.M. (1992) Triplex formation prevents Sp1 binding to the dihydrofolate reductase promoter.	bind
26951	1	8167	6	13	NULL	NULL	NULL	p53	GP		bind		sequence specifically			DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_5207_s_415	11812854	40       Gu,W. and Roeder,R.G. (1997) Activation of p53 sequence-specific DNA binding by acetylation of the p53 C-terminal domain.	bind
26952	2	8167	6	13	NULL	NULL	NULL	p53	GP	acetylation of	activates			C-terminal domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_5207_s_415	11812854	40       Gu,W. and Roeder,R.G. (1997) Activation of p53 sequence-specific DNA binding by acetylation of the p53 C-terminal domain.	bind
32703	1	8167	7	10	NULL	0	NULL	 p53	NULL		bind	NULL	sequence specifically			DNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_5207_s_415	11812854	40       Gu,W. and Roeder,R.G. (1997) Activation of p53 sequence-specific DNA binding by acetylation of the p53 C-terminal domain.	bind
32705	2	8167	7	10	NULL	0	NULL	p53	NULL		undergoes	NULL		C-terminal domain		acetylation	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_5207_s_415	11812854	40       Gu,W. and Roeder,R.G. (1997) Activation of p53 sequence-specific DNA binding by acetylation of the p53 C-terminal domain.	bind
32706	3	8167	7	10	NULL	0	NULL	statement 2	NULL		activates	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_5207_s_415	11812854	40       Gu,W. and Roeder,R.G. (1997) Activation of p53 sequence-specific DNA binding by acetylation of the p53 C-terminal domain.	bind
26953	1	8168	6	13	NULL	NULL	NULL	U2AF	GP		is required for					U2 snRNP	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1741_s_328	11292847	40       Ruskin,B., Zamore,P.D. and Green,M.R. (1988) A factor, U2AF, is required for U2 snRNP binding and splicing complex assembly.	bind
26954	2	8168	6	13	NULL	NULL	NULL	U2AF	GP		is required for					splicing complex	GP	assembly of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1741_s_328	11292847	40       Ruskin,B., Zamore,P.D. and Green,M.R. (1988) A factor, U2AF, is required for U2 snRNP binding and splicing complex assembly.	bind
32713	1	8168	7	NULL	NULL	0	NULL	U2	NULL		bind	NULL				SnRNP	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1741_s_328	11292847	40       Ruskin,B., Zamore,P.D. and Green,M.R. (1988) A factor, U2AF, is required for U2 snRNP binding and splicing complex assembly.	bind
32714	2	8168	7	NULL	NULL	0	NULL	U2AF	NULL		is required for	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1741_s_328	11292847	40       Ruskin,B., Zamore,P.D. and Green,M.R. (1988) A factor, U2AF, is required for U2 snRNP binding and splicing complex assembly.	bind
32715	3	8168	7	NULL	NULL	0	NULL	U2AF	NULL		is required for	NULL				splicing complex	NULL	assembly of			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1741_s_328	11292847	40       Ruskin,B., Zamore,P.D. and Green,M.R. (1988) A factor, U2AF, is required for U2 snRNP binding and splicing complex assembly.	bind
26955	1	8169	6	13	NULL	NULL	NULL	LDL	GP		bind		may			GPIIb	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_377_s_163	7749848	40  Although ligand blotting experiments reveal that LDL and HDL may bind to GPIIb and GPIIIa, respectively, 15  only LDL seems to increase exposure of fibrinogen binding sites on ADP-stimulated GFPs. 46  Van Willigen et al 46  have shown that exposure of the GPIIb-IIIa complex, the so-called fibrinogen receptor, is not mediated by formation of proaggregatory eicosanoids, ie, PGG2/H2 and TXA2.	bind
26956	2	8169	6	13	NULL	NULL	NULL	HDL	GP		bind		may			GPIIIa	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_377_s_163	7749848	40  Although ligand blotting experiments reveal that LDL and HDL may bind to GPIIb and GPIIIa, respectively, 15  only LDL seems to increase exposure of fibrinogen binding sites on ADP-stimulated GFPs. 46  Van Willigen et al 46  have shown that exposure of the GPIIb-IIIa complex, the so-called fibrinogen receptor, is not mediated by formation of proaggregatory eicosanoids, ie, PGG2/H2 and TXA2.	bind
27035	3	8169	6	13	NULL	NULL	NULL	LDL	GP		increase		may			GFP	GP	exposure of;; ADP stimulated	fibrinogen binding sites		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_377_s_163	7749848	40  Although ligand blotting experiments reveal that LDL and HDL may bind to GPIIb and GPIIIa, respectively, 15  only LDL seems to increase exposure of fibrinogen binding sites on ADP-stimulated GFPs. 46  Van Willigen et al 46  have shown that exposure of the GPIIb-IIIa complex, the so-called fibrinogen receptor, is not mediated by formation of proaggregatory eicosanoids, ie, PGG2/H2 and TXA2.	bind
27036	4	8169	6	13	NULL	NULL	NULL	GPIIb-IIIa complex	GP		is a type of					fibrinogen receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_377_s_163	7749848	40  Although ligand blotting experiments reveal that LDL and HDL may bind to GPIIb and GPIIIa, respectively, 15  only LDL seems to increase exposure of fibrinogen binding sites on ADP-stimulated GFPs. 46  Van Willigen et al 46  have shown that exposure of the GPIIb-IIIa complex, the so-called fibrinogen receptor, is not mediated by formation of proaggregatory eicosanoids, ie, PGG2/H2 and TXA2.	bind
27037	5	8169	6	13	NULL	NULL	NULL	GPIIb-IIIa complex	GP	exposure of	is not mediated by					eicosanoids	Chemical	formation of;; proaggregatory			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_377_s_163	7749848	40  Although ligand blotting experiments reveal that LDL and HDL may bind to GPIIb and GPIIIa, respectively, 15  only LDL seems to increase exposure of fibrinogen binding sites on ADP-stimulated GFPs. 46  Van Willigen et al 46  have shown that exposure of the GPIIb-IIIa complex, the so-called fibrinogen receptor, is not mediated by formation of proaggregatory eicosanoids, ie, PGG2/H2 and TXA2.	bind
27038	6	8169	6	13	NULL	NULL	NULL	PGG2/H2	Chemical		is a type of					proaggregatory eicosanoid	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_377_s_163	7749848	40  Although ligand blotting experiments reveal that LDL and HDL may bind to GPIIb and GPIIIa, respectively, 15  only LDL seems to increase exposure of fibrinogen binding sites on ADP-stimulated GFPs. 46  Van Willigen et al 46  have shown that exposure of the GPIIb-IIIa complex, the so-called fibrinogen receptor, is not mediated by formation of proaggregatory eicosanoids, ie, PGG2/H2 and TXA2.	bind
27055	7	8169	6	13	NULL	NULL	NULL	TXA2	Chemical		is a type of					proaggregatory eicosanoid	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_377_s_163	7749848	40  Although ligand blotting experiments reveal that LDL and HDL may bind to GPIIb and GPIIIa, respectively, 15  only LDL seems to increase exposure of fibrinogen binding sites on ADP-stimulated GFPs. 46  Van Willigen et al 46  have shown that exposure of the GPIIb-IIIa complex, the so-called fibrinogen receptor, is not mediated by formation of proaggregatory eicosanoids, ie, PGG2/H2 and TXA2.	bind
32716	1	8169	7	NULL	NULL	0	NULL	LDL 	NULL		bind	NULL	may			GPIIb	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_377_s_163	7749848	40  Although ligand blotting experiments reveal that LDL and HDL may bind to GPIIb and GPIIIa, respectively, 15  only LDL seems to increase exposure of fibrinogen binding sites on ADP-stimulated GFPs. 46  Van Willigen et al 46  have shown that exposure of the GPIIb-IIIa complex, the so-called fibrinogen receptor, is not mediated by formation of proaggregatory eicosanoids, ie, PGG2/H2 and TXA2.	bind
32717	2	8169	7	NULL	NULL	0	NULL	HDL	NULL		bind	NULL	may			GPIIIa	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_377_s_163	7749848	40  Although ligand blotting experiments reveal that LDL and HDL may bind to GPIIb and GPIIIa, respectively, 15  only LDL seems to increase exposure of fibrinogen binding sites on ADP-stimulated GFPs. 46  Van Willigen et al 46  have shown that exposure of the GPIIb-IIIa complex, the so-called fibrinogen receptor, is not mediated by formation of proaggregatory eicosanoids, ie, PGG2/H2 and TXA2.	bind
32718	3	8169	7	NULL	NULL	0	NULL	ADP	NULL		stimulate	NULL				GFPs	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_377_s_163	7749848	40  Although ligand blotting experiments reveal that LDL and HDL may bind to GPIIb and GPIIIa, respectively, 15  only LDL seems to increase exposure of fibrinogen binding sites on ADP-stimulated GFPs. 46  Van Willigen et al 46  have shown that exposure of the GPIIb-IIIa complex, the so-called fibrinogen receptor, is not mediated by formation of proaggregatory eicosanoids, ie, PGG2/H2 and TXA2.	bind
32719	4	8169	7	10	NULL	0	NULL	LDL	NULL		increase	NULL				GFPs	NULL	exposure of;;ADP-stimulated	fibrinogen binding sites		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_377_s_163	7749848	40  Although ligand blotting experiments reveal that LDL and HDL may bind to GPIIb and GPIIIa, respectively, 15  only LDL seems to increase exposure of fibrinogen binding sites on ADP-stimulated GFPs. 46  Van Willigen et al 46  have shown that exposure of the GPIIb-IIIa complex, the so-called fibrinogen receptor, is not mediated by formation of proaggregatory eicosanoids, ie, PGG2/H2 and TXA2.	bind
32720	5	8169	7	NULL	NULL	0	NULL	 GPIIb-IIIa complex	NULL		is a type of	NULL				fibrinogen receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_377_s_163	7749848	40  Although ligand blotting experiments reveal that LDL and HDL may bind to GPIIb and GPIIIa, respectively, 15  only LDL seems to increase exposure of fibrinogen binding sites on ADP-stimulated GFPs. 46  Van Willigen et al 46  have shown that exposure of the GPIIb-IIIa complex, the so-called fibrinogen receptor, is not mediated by formation of proaggregatory eicosanoids, ie, PGG2/H2 and TXA2.	bind
32721	6	8169	7	NULL	NULL	0	NULL	 GPIIb-IIIa complex	NULL	exposure of	is not mediated by	NULL				PGG2/H2	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_377_s_163	7749848	40  Although ligand blotting experiments reveal that LDL and HDL may bind to GPIIb and GPIIIa, respectively, 15  only LDL seems to increase exposure of fibrinogen binding sites on ADP-stimulated GFPs. 46  Van Willigen et al 46  have shown that exposure of the GPIIb-IIIa complex, the so-called fibrinogen receptor, is not mediated by formation of proaggregatory eicosanoids, ie, PGG2/H2 and TXA2.	bind
32722	7	8169	7	NULL	NULL	0	NULL	GPIIb-IIIa complex	NULL	exposure of	is not mediated by	NULL				TXA2	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_377_s_163	7749848	40  Although ligand blotting experiments reveal that LDL and HDL may bind to GPIIb and GPIIIa, respectively, 15  only LDL seems to increase exposure of fibrinogen binding sites on ADP-stimulated GFPs. 46  Van Willigen et al 46  have shown that exposure of the GPIIb-IIIa complex, the so-called fibrinogen receptor, is not mediated by formation of proaggregatory eicosanoids, ie, PGG2/H2 and TXA2.	bind
32723	8	8169	7	NULL	NULL	0	NULL	PGG2/H2	NULL		is a type of	NULL				proaggregatory eicosanoids	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_377_s_163	7749848	40  Although ligand blotting experiments reveal that LDL and HDL may bind to GPIIb and GPIIIa, respectively, 15  only LDL seems to increase exposure of fibrinogen binding sites on ADP-stimulated GFPs. 46  Van Willigen et al 46  have shown that exposure of the GPIIb-IIIa complex, the so-called fibrinogen receptor, is not mediated by formation of proaggregatory eicosanoids, ie, PGG2/H2 and TXA2.	bind
32724	9	8169	7	NULL	NULL	0	NULL	TXA2	NULL		is a type of	NULL				proaggregatory eicosanoids	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_377_s_163	7749848	40  Although ligand blotting experiments reveal that LDL and HDL may bind to GPIIb and GPIIIa, respectively, 15  only LDL seems to increase exposure of fibrinogen binding sites on ADP-stimulated GFPs. 46  Van Willigen et al 46  have shown that exposure of the GPIIb-IIIa complex, the so-called fibrinogen receptor, is not mediated by formation of proaggregatory eicosanoids, ie, PGG2/H2 and TXA2.	bind
27508	1	8170	6	13	NULL	NULL	NULL	Rel A	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_205_s_322	11786414	40  As the DNA binding of RelA and p50 may also be disturbed by their hypophosphorylation 39 and as different NF-kappaB-inducing stimuli may cause phosphorylation of NF-kappaB proteins at unique sites, 41, 42  which possibly differentially affects their DNA binding, selective inhibition of RelA or p50 phosphorylation could be the mechanism by which SS blocks NF-kappaB DNA binding in human testicular cells under the conditions induced in the present model.	bind
27509	2	8170	6	13	NULL	NULL	NULL	p50	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_205_s_322	11786414	40  As the DNA binding of RelA and p50 may also be disturbed by their hypophosphorylation 39 and as different NF-kappaB-inducing stimuli may cause phosphorylation of NF-kappaB proteins at unique sites, 41, 42  which possibly differentially affects their DNA binding, selective inhibition of RelA or p50 phosphorylation could be the mechanism by which SS blocks NF-kappaB DNA binding in human testicular cells under the conditions induced in the present model.	bind
27510	3	8170	6	13	NULL	NULL	NULL	Rel A	GP	hyperphosphorylation of	disturb		may			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_205_s_322	11786414	40  As the DNA binding of RelA and p50 may also be disturbed by their hypophosphorylation 39 and as different NF-kappaB-inducing stimuli may cause phosphorylation of NF-kappaB proteins at unique sites, 41, 42  which possibly differentially affects their DNA binding, selective inhibition of RelA or p50 phosphorylation could be the mechanism by which SS blocks NF-kappaB DNA binding in human testicular cells under the conditions induced in the present model.	bind
27511	4	8170	6	13	NULL	NULL	NULL	p50	GP	hyperphosphorylation of	disturb		may			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_205_s_322	11786414	40  As the DNA binding of RelA and p50 may also be disturbed by their hypophosphorylation 39 and as different NF-kappaB-inducing stimuli may cause phosphorylation of NF-kappaB proteins at unique sites, 41, 42  which possibly differentially affects their DNA binding, selective inhibition of RelA or p50 phosphorylation could be the mechanism by which SS blocks NF-kappaB DNA binding in human testicular cells under the conditions induced in the present model.	bind
27512	5	8170	6	13	NULL	NULL	NULL	NF-kappaB	GP		bind					DNA	NucleicAcid				NULL	human testicular cells	NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_205_s_322	11786414	40  As the DNA binding of RelA and p50 may also be disturbed by their hypophosphorylation 39 and as different NF-kappaB-inducing stimuli may cause phosphorylation of NF-kappaB proteins at unique sites, 41, 42  which possibly differentially affects their DNA binding, selective inhibition of RelA or p50 phosphorylation could be the mechanism by which SS blocks NF-kappaB DNA binding in human testicular cells under the conditions induced in the present model.	bind
27513	6	8170	6	13	NULL	NULL	NULL	SS	Chemical		blocks					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_205_s_322	11786414	40  As the DNA binding of RelA and p50 may also be disturbed by their hypophosphorylation 39 and as different NF-kappaB-inducing stimuli may cause phosphorylation of NF-kappaB proteins at unique sites, 41, 42  which possibly differentially affects their DNA binding, selective inhibition of RelA or p50 phosphorylation could be the mechanism by which SS blocks NF-kappaB DNA binding in human testicular cells under the conditions induced in the present model.	bind
27514	7	8170	6	13	NULL	NULL	NULL	Rel A	GP	selective inhibition of;;phosphorylation	is mechanism for		could			statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_205_s_322	11786414	40  As the DNA binding of RelA and p50 may also be disturbed by their hypophosphorylation 39 and as different NF-kappaB-inducing stimuli may cause phosphorylation of NF-kappaB proteins at unique sites, 41, 42  which possibly differentially affects their DNA binding, selective inhibition of RelA or p50 phosphorylation could be the mechanism by which SS blocks NF-kappaB DNA binding in human testicular cells under the conditions induced in the present model.	bind
27515	8	8170	6	13	NULL	NULL	NULL	p50	GP	selective inhibition of;;phosphorylation	is mechanism for		could			statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_205_s_322	11786414	40  As the DNA binding of RelA and p50 may also be disturbed by their hypophosphorylation 39 and as different NF-kappaB-inducing stimuli may cause phosphorylation of NF-kappaB proteins at unique sites, 41, 42  which possibly differentially affects their DNA binding, selective inhibition of RelA or p50 phosphorylation could be the mechanism by which SS blocks NF-kappaB DNA binding in human testicular cells under the conditions induced in the present model.	bind
32725	1	8170	7	NULL	NULL	0	NULL	RelA 	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_1_205_s_322	11786414	40  As the DNA binding of RelA and p50 may also be disturbed by their hypophosphorylation 39 and as different NF-kappaB-inducing stimuli may cause phosphorylation of NF-kappaB proteins at unique sites, 41, 42  which possibly differentially affects their DNA binding, selective inhibition of RelA or p50 phosphorylation could be the mechanism by which SS blocks NF-kappaB DNA binding in human testicular cells under the conditions induced in the present model.	bind
32726	2	8170	7	NULL	NULL	0	NULL	p50	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_1_205_s_322	11786414	40  As the DNA binding of RelA and p50 may also be disturbed by their hypophosphorylation 39 and as different NF-kappaB-inducing stimuli may cause phosphorylation of NF-kappaB proteins at unique sites, 41, 42  which possibly differentially affects their DNA binding, selective inhibition of RelA or p50 phosphorylation could be the mechanism by which SS blocks NF-kappaB DNA binding in human testicular cells under the conditions induced in the present model.	bind
32727	3	8170	7	NULL	NULL	0	NULL	statement 1	NULL		be disturbed by	NULL	may			hypophosphorylation 	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_205_s_322	11786414	40  As the DNA binding of RelA and p50 may also be disturbed by their hypophosphorylation 39 and as different NF-kappaB-inducing stimuli may cause phosphorylation of NF-kappaB proteins at unique sites, 41, 42  which possibly differentially affects their DNA binding, selective inhibition of RelA or p50 phosphorylation could be the mechanism by which SS blocks NF-kappaB DNA binding in human testicular cells under the conditions induced in the present model.	bind
32728	4	8170	7	NULL	NULL	0	NULL	statement 2	NULL		 be disturbed by	NULL	may			hypophosphorylation 	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_205_s_322	11786414	40  As the DNA binding of RelA and p50 may also be disturbed by their hypophosphorylation 39 and as different NF-kappaB-inducing stimuli may cause phosphorylation of NF-kappaB proteins at unique sites, 41, 42  which possibly differentially affects their DNA binding, selective inhibition of RelA or p50 phosphorylation could be the mechanism by which SS blocks NF-kappaB DNA binding in human testicular cells under the conditions induced in the present model.	bind
32729	5	8170	7	NULL	NULL	0	NULL	stimuli	NULL		induce	NULL				NF-kappaB	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_1_205_s_322	11786414	40  As the DNA binding of RelA and p50 may also be disturbed by their hypophosphorylation 39 and as different NF-kappaB-inducing stimuli may cause phosphorylation of NF-kappaB proteins at unique sites, 41, 42  which possibly differentially affects their DNA binding, selective inhibition of RelA or p50 phosphorylation could be the mechanism by which SS blocks NF-kappaB DNA binding in human testicular cells under the conditions induced in the present model.	bind
32730	6	8170	7	NULL	NULL	0	NULL	statement 5	NULL		cause	NULL	may			NF-kappaB proteins	NULL	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_1_205_s_322	11786414	40  As the DNA binding of RelA and p50 may also be disturbed by their hypophosphorylation 39 and as different NF-kappaB-inducing stimuli may cause phosphorylation of NF-kappaB proteins at unique sites, 41, 42  which possibly differentially affects their DNA binding, selective inhibition of RelA or p50 phosphorylation could be the mechanism by which SS blocks NF-kappaB DNA binding in human testicular cells under the conditions induced in the present model.	bind
32731	7	8170	7	NULL	NULL	0	NULL	NF-kappaB	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_1_205_s_322	11786414	40  As the DNA binding of RelA and p50 may also be disturbed by their hypophosphorylation 39 and as different NF-kappaB-inducing stimuli may cause phosphorylation of NF-kappaB proteins at unique sites, 41, 42  which possibly differentially affects their DNA binding, selective inhibition of RelA or p50 phosphorylation could be the mechanism by which SS blocks NF-kappaB DNA binding in human testicular cells under the conditions induced in the present model.	bind
32732	8	8170	7	NULL	NULL	0	NULL	statement 6	NULL		affect	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_1_205_s_322	11786414	40  As the DNA binding of RelA and p50 may also be disturbed by their hypophosphorylation 39 and as different NF-kappaB-inducing stimuli may cause phosphorylation of NF-kappaB proteins at unique sites, 41, 42  which possibly differentially affects their DNA binding, selective inhibition of RelA or p50 phosphorylation could be the mechanism by which SS blocks NF-kappaB DNA binding in human testicular cells under the conditions induced in the present model.	bind
32733	9	8170	7	NULL	NULL	0	NULL	SS 	NULL		blocks	NULL				statement 7	NULL				NULL	human testicular cells	0	NULL	NULL	NULL	gw60_amjpathol_160_1_205_s_322	11786414	40  As the DNA binding of RelA and p50 may also be disturbed by their hypophosphorylation 39 and as different NF-kappaB-inducing stimuli may cause phosphorylation of NF-kappaB proteins at unique sites, 41, 42  which possibly differentially affects their DNA binding, selective inhibition of RelA or p50 phosphorylation could be the mechanism by which SS blocks NF-kappaB DNA binding in human testicular cells under the conditions induced in the present model.	bind
32734	10	8170	7	10	NULL	0	NULL	RelA	NULL	inhibition of;;phosphorylation of	is the mechanism for	NULL				statement 9	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_205_s_322	11786414	40  As the DNA binding of RelA and p50 may also be disturbed by their hypophosphorylation 39 and as different NF-kappaB-inducing stimuli may cause phosphorylation of NF-kappaB proteins at unique sites, 41, 42  which possibly differentially affects their DNA binding, selective inhibition of RelA or p50 phosphorylation could be the mechanism by which SS blocks NF-kappaB DNA binding in human testicular cells under the conditions induced in the present model.	bind
32735	11	8170	7	10	NULL	0	NULL	p50	NULL	inhibition of;;phosphorylation of	is the mechanism for	NULL				statement 9	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_205_s_322	11786414	40  As the DNA binding of RelA and p50 may also be disturbed by their hypophosphorylation 39 and as different NF-kappaB-inducing stimuli may cause phosphorylation of NF-kappaB proteins at unique sites, 41, 42  which possibly differentially affects their DNA binding, selective inhibition of RelA or p50 phosphorylation could be the mechanism by which SS blocks NF-kappaB DNA binding in human testicular cells under the conditions induced in the present model.	bind
27059	1	8171	6	13	NULL	NULL	NULL	DEGR-VIIa	GP		bind					tissue factor	GP				NULL	cell surface	NULL	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_254	7586275	40  DEGR-VIIa binds tissue factor with fivefold to sevenfold more affinity than native factor VIIa in the cell surface chromogenic assay, rendering the DEGR-VIIa - tissue factor complex enzymatically inactive and thus inhibiting the conversion of factor IX to IXa and factor X to Xa.	bind
27060	2	8171	6	13	NULL	NULL	NULL	factor VIIa	GP	native	bind					tissue factor	GP				NULL	cell surface	NULL	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_254	7586275	40  DEGR-VIIa binds tissue factor with fivefold to sevenfold more affinity than native factor VIIa in the cell surface chromogenic assay, rendering the DEGR-VIIa - tissue factor complex enzymatically inactive and thus inhibiting the conversion of factor IX to IXa and factor X to Xa.	bind
27061	3	8171	6	13	NULL	NULL	NULL	statement 1	Process	affinity of	is higher than					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_254	7586275	40  DEGR-VIIa binds tissue factor with fivefold to sevenfold more affinity than native factor VIIa in the cell surface chromogenic assay, rendering the DEGR-VIIa - tissue factor complex enzymatically inactive and thus inhibiting the conversion of factor IX to IXa and factor X to Xa.	bind
27062	4	8171	6	13	NULL	NULL	NULL	factor IX	GP		is converted to					factor IXa	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_254	7586275	40  DEGR-VIIa binds tissue factor with fivefold to sevenfold more affinity than native factor VIIa in the cell surface chromogenic assay, rendering the DEGR-VIIa - tissue factor complex enzymatically inactive and thus inhibiting the conversion of factor IX to IXa and factor X to Xa.	bind
27063	5	8171	6	13	NULL	NULL	NULL	factor X	GP		is converted to					factor Xa	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_254	7586275	40  DEGR-VIIa binds tissue factor with fivefold to sevenfold more affinity than native factor VIIa in the cell surface chromogenic assay, rendering the DEGR-VIIa - tissue factor complex enzymatically inactive and thus inhibiting the conversion of factor IX to IXa and factor X to Xa.	bind
27064	6	8171	6	13	NULL	NULL	NULL	statement 1	Process		inactivates					DEGR-VIIa - tissue factor complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_254	7586275	40  DEGR-VIIa binds tissue factor with fivefold to sevenfold more affinity than native factor VIIa in the cell surface chromogenic assay, rendering the DEGR-VIIa - tissue factor complex enzymatically inactive and thus inhibiting the conversion of factor IX to IXa and factor X to Xa.	bind
27065	7	8171	6	13	NULL	NULL	NULL	statement 6	Process		inhibits					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_254	7586275	40  DEGR-VIIa binds tissue factor with fivefold to sevenfold more affinity than native factor VIIa in the cell surface chromogenic assay, rendering the DEGR-VIIa - tissue factor complex enzymatically inactive and thus inhibiting the conversion of factor IX to IXa and factor X to Xa.	bind
27066	8	8171	6	13	NULL	NULL	NULL	statement 6	Process		inhibits					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_254	7586275	40  DEGR-VIIa binds tissue factor with fivefold to sevenfold more affinity than native factor VIIa in the cell surface chromogenic assay, rendering the DEGR-VIIa - tissue factor complex enzymatically inactive and thus inhibiting the conversion of factor IX to IXa and factor X to Xa.	bind
32736	1	8171	7	NULL	NULL	0	NULL	DEGR-VIIa	NULL		binds	NULL				tissue factor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_254	7586275	40  DEGR-VIIa binds tissue factor with fivefold to sevenfold more affinity than native factor VIIa in the cell surface chromogenic assay, rendering the DEGR-VIIa - tissue factor complex enzymatically inactive and thus inhibiting the conversion of factor IX to IXa and factor X to Xa.	bind
32737	2	8171	7	NULL	NULL	0	NULL	 factor VIIa	NULL	native	binds	NULL				tissue factor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_254	7586275	40  DEGR-VIIa binds tissue factor with fivefold to sevenfold more affinity than native factor VIIa in the cell surface chromogenic assay, rendering the DEGR-VIIa - tissue factor complex enzymatically inactive and thus inhibiting the conversion of factor IX to IXa and factor X to Xa.	bind
32738	3	8171	7	NULL	NULL	0	NULL	statement 1	NULL	affinity of	is higher than	NULL				statement 2	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_254	7586275	40  DEGR-VIIa binds tissue factor with fivefold to sevenfold more affinity than native factor VIIa in the cell surface chromogenic assay, rendering the DEGR-VIIa - tissue factor complex enzymatically inactive and thus inhibiting the conversion of factor IX to IXa and factor X to Xa.	bind
32739	4	8171	7	NULL	NULL	0	NULL	DEGR-VIIa - tissue factor complex 	NULL		is inactive as	NULL				enzyme	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_254	7586275	40  DEGR-VIIa binds tissue factor with fivefold to sevenfold more affinity than native factor VIIa in the cell surface chromogenic assay, rendering the DEGR-VIIa - tissue factor complex enzymatically inactive and thus inhibiting the conversion of factor IX to IXa and factor X to Xa.	bind
32740	5	8171	7	NULL	NULL	0	NULL	factor IX	NULL		converts to	NULL				factor IXa	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_254	7586275	40  DEGR-VIIa binds tissue factor with fivefold to sevenfold more affinity than native factor VIIa in the cell surface chromogenic assay, rendering the DEGR-VIIa - tissue factor complex enzymatically inactive and thus inhibiting the conversion of factor IX to IXa and factor X to Xa.	bind
32741	6	8171	7	NULL	NULL	0	NULL	factor X	NULL		converts to	NULL				factor Xa	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_254	7586275	40  DEGR-VIIa binds tissue factor with fivefold to sevenfold more affinity than native factor VIIa in the cell surface chromogenic assay, rendering the DEGR-VIIa - tissue factor complex enzymatically inactive and thus inhibiting the conversion of factor IX to IXa and factor X to Xa.	bind
32742	7	8171	7	NULL	NULL	0	NULL	statement 4	NULL		inhibits	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_254	7586275	40  DEGR-VIIa binds tissue factor with fivefold to sevenfold more affinity than native factor VIIa in the cell surface chromogenic assay, rendering the DEGR-VIIa - tissue factor complex enzymatically inactive and thus inhibiting the conversion of factor IX to IXa and factor X to Xa.	bind
32743	8	8171	7	NULL	NULL	0	NULL	statement 4	NULL		inhibits	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_254	7586275	40  DEGR-VIIa binds tissue factor with fivefold to sevenfold more affinity than native factor VIIa in the cell surface chromogenic assay, rendering the DEGR-VIIa - tissue factor complex enzymatically inactive and thus inhibiting the conversion of factor IX to IXa and factor X to Xa.	bind
27068	1	8172	6	13	NULL	NULL	NULL	anti-membrane glycoprotein MAb	GP		bind					SMC	Cell				NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_6_1515_s_130	9118520	40  However, this possibility was unlikely because anti-membrane glycoprotein MAb, which binds SMC surface antigen, did not affect IH.	bind
27069	2	8172	6	13	NULL	NULL	NULL	anti-membrane glycoprotein MAb	GP		did not affect					IH	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_6_1515_s_130	9118520	40  However, this possibility was unlikely because anti-membrane glycoprotein MAb, which binds SMC surface antigen, did not affect IH.	bind
46605	3	8172	6	10	NULL	0	NULL	SMC	NULL		is a type of	NULL				surface antigen	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_95_6_1515_s_130	9118520	40  However, this possibility was unlikely because anti-membrane glycoprotein MAb, which binds SMC surface antigen, did not affect IH.	bind
32744	1	8172	7	NULL	NULL	0	NULL	anti-membrane glycoprotein MAb	NULL		binds	NULL				SMC	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_95_6_1515_s_130	9118520	40  However, this possibility was unlikely because anti-membrane glycoprotein MAb, which binds SMC surface antigen, did not affect IH.	bind
32745	2	8172	7	NULL	NULL	0	NULL	anti-membrane glycoprotein MAb	NULL		does not affect	NULL				IH	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_95_6_1515_s_130	9118520	40  However, this possibility was unlikely because anti-membrane glycoprotein MAb, which binds SMC surface antigen, did not affect IH.	bind
32746	3	8172	7	NULL	NULL	0	NULL	SMC	NULL		is a type of	NULL				surface antigen	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_95_6_1515_s_130	9118520	40  However, this possibility was unlikely because anti-membrane glycoprotein MAb, which binds SMC surface antigen, did not affect IH.	bind
27071	1	8173	6	13	NULL	NULL	NULL	factor VIII	GP		bind					von Willebrand factor	GP				NULL	plasma	NULL	NULL	NULL	NULL	gw60_circulation_96_4_1102_s_141	9286936	40  In women, factor VIII was also positively associated with CHD incidence, which might be expected because factor VIII is bound to von Willebrand factor in plasma and there is a correlation of 0.71 between these two factors.	bind
27072	2	8173	6	13	NULL	NULL	NULL	factor VIII	GP		is associated with		positively			CHD	MedicalFinding	incidence of 			NULL	women	NULL	NULL	NULL	NULL	gw60_circulation_96_4_1102_s_141	9286936	40  In women, factor VIII was also positively associated with CHD incidence, which might be expected because factor VIII is bound to von Willebrand factor in plasma and there is a correlation of 0.71 between these two factors.	bind
32747	1	8173	7	10	NULL	0	NULL	factor VIII			associated with		positively			CHD		incidence of			NULL	women	NULL	NULL	NULL	NULL	gw60_circulation_96_4_1102_s_141	9286936	40  In women, factor VIII was also positively associated with CHD incidence, which might be expected because factor VIII is bound to von Willebrand factor in plasma and there is a correlation of 0.71 between these two factors.	bind
32748	2	8173	7	NULL	NULL	0	NULL	factor VIII	NULL		bind	NULL				von Willebrand factor	NULL				NULL	plasma	0	NULL	NULL	NULL	gw60_circulation_96_4_1102_s_141	9286936	40  In women, factor VIII was also positively associated with CHD incidence, which might be expected because factor VIII is bound to von Willebrand factor in plasma and there is a correlation of 0.71 between these two factors.	bind
27073	1	8174	6	13	NULL	NULL	NULL	UPA	GP	mouse	bind		specifically			UPAR	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_693_s_52	9598826	40  Moreover, comparison of the species-specific binding of UPA to UPAR with the amino acid sequence of the presumed binding sites in mouse, pig, and human UPA reveals that this species specificity must be mediated by very minor differences in amino acid sequence, most likely at positions 22, 27, 29, and 30, which are structurally close to each other 39  and wherein human and murine UPA have different amino acid residues.	bind
27696	2	8174	6	13	NULL	NULL	NULL	UPA	GP	pig	bind					UPAR	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_693_s_52	9598826	40  Moreover, comparison of the species-specific binding of UPA to UPAR with the amino acid sequence of the presumed binding sites in mouse, pig, and human UPA reveals that this species specificity must be mediated by very minor differences in amino acid sequence, most likely at positions 22, 27, 29, and 30, which are structurally close to each other 39  and wherein human and murine UPA have different amino acid residues.	bind
27697	3	8174	6	13	NULL	NULL	NULL	UPA	GP	human	bind					UPAR	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_693_s_52	9598826	40  Moreover, comparison of the species-specific binding of UPA to UPAR with the amino acid sequence of the presumed binding sites in mouse, pig, and human UPA reveals that this species specificity must be mediated by very minor differences in amino acid sequence, most likely at positions 22, 27, 29, and 30, which are structurally close to each other 39  and wherein human and murine UPA have different amino acid residues.	bind
32749	1	8174	7	NULL	NULL	0	NULL	UPA	NULL	mouse	binds	NULL				UPAR	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_693_s_52	9598826	40  Moreover, comparison of the species-specific binding of UPA to UPAR with the amino acid sequence of the presumed binding sites in mouse, pig, and human UPA reveals that this species specificity must be mediated by very minor differences in amino acid sequence, most likely at positions 22, 27, 29, and 30, which are structurally close to each other 39  and wherein human and murine UPA have different amino acid residues.	bind
32750	2	8174	7	NULL	NULL	0	NULL	UPA	NULL	pig	binds	NULL				UPAR	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_693_s_52	9598826	40  Moreover, comparison of the species-specific binding of UPA to UPAR with the amino acid sequence of the presumed binding sites in mouse, pig, and human UPA reveals that this species specificity must be mediated by very minor differences in amino acid sequence, most likely at positions 22, 27, 29, and 30, which are structurally close to each other 39  and wherein human and murine UPA have different amino acid residues.	bind
32751	3	8174	7	NULL	NULL	0	NULL	UPA	NULL	human	binds	NULL				UPAR	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_693_s_52	9598826	40  Moreover, comparison of the species-specific binding of UPA to UPAR with the amino acid sequence of the presumed binding sites in mouse, pig, and human UPA reveals that this species specificity must be mediated by very minor differences in amino acid sequence, most likely at positions 22, 27, 29, and 30, which are structurally close to each other 39  and wherein human and murine UPA have different amino acid residues.	bind
32752	4	8174	7	NULL	NULL	0	NULL	species specificity	NULL		is mediated by	NULL				UPA	NULL		aminoacid 22		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_693_s_52	9598826	40  Moreover, comparison of the species-specific binding of UPA to UPAR with the amino acid sequence of the presumed binding sites in mouse, pig, and human UPA reveals that this species specificity must be mediated by very minor differences in amino acid sequence, most likely at positions 22, 27, 29, and 30, which are structurally close to each other 39  and wherein human and murine UPA have different amino acid residues.	bind
32753	5	8174	7	NULL	NULL	0	NULL	species specificity	NULL		is mediated by	NULL				UPA	NULL		amino acid 27		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_693_s_52	9598826	40  Moreover, comparison of the species-specific binding of UPA to UPAR with the amino acid sequence of the presumed binding sites in mouse, pig, and human UPA reveals that this species specificity must be mediated by very minor differences in amino acid sequence, most likely at positions 22, 27, 29, and 30, which are structurally close to each other 39  and wherein human and murine UPA have different amino acid residues.	bind
32754	6	8174	7	NULL	NULL	0	NULL	species specificity	NULL		is mediated by	NULL				UPA	NULL		amino acid 29		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_693_s_52	9598826	40  Moreover, comparison of the species-specific binding of UPA to UPAR with the amino acid sequence of the presumed binding sites in mouse, pig, and human UPA reveals that this species specificity must be mediated by very minor differences in amino acid sequence, most likely at positions 22, 27, 29, and 30, which are structurally close to each other 39  and wherein human and murine UPA have different amino acid residues.	bind
32755	7	8174	7	NULL	NULL	0	NULL	species specificity	NULL		is mediated by	NULL				UPA	NULL		amino acid 30		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_693_s_52	9598826	40  Moreover, comparison of the species-specific binding of UPA to UPAR with the amino acid sequence of the presumed binding sites in mouse, pig, and human UPA reveals that this species specificity must be mediated by very minor differences in amino acid sequence, most likely at positions 22, 27, 29, and 30, which are structurally close to each other 39  and wherein human and murine UPA have different amino acid residues.	bind
27074	1	8175	6	13	NULL	NULL	NULL	RACK1	GP		bind					Src	GP				NULL	cells treated with PMA	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_23_20346_s_281	11279199	40 and  41), we detected little increase in binding of RACK1 and Src after treating cells with PMA for 15 min (Fig.  8,  A ( lane 6) and  B ( lanes 4 and  7)).	bind
32996	1	8175	7	NULL	NULL	0	NULL	 RACK1	NULL		bind	NULL				Src	NULL				NULL	cells treated with PMA	0	NULL	NULL	NULL	gw60_jbiolchem_276_23_20346_s_281	11279199	40 and  41), we detected little increase in binding of RACK1 and Src after treating cells with PMA for 15 min (Fig.  8,  A ( lane 6) and  B ( lanes 4 and  7)).	bind
27075	1	8176	6	13	NULL	NULL	NULL	CaN	GP		bind					AKAP	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_7_866_s_115	15087426	40 From their studies, the authors concluded not only that AKAP79, PKA, CaN, and membrane-associated guanylate kinase are assembled in a macromolecular complex in intact cells but also that, by FRET imaging, CaN and PKA bind to AKAP 79 within 5 nm of each other, thus extending our understanding of the level of molecular compartmentation of signaling proteins that is made possible by scaffolding proteins.	bind
27076	2	8176	6	13	NULL	NULL	NULL	PKA	GP		bind					AKAP	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_7_866_s_115	15087426	40 From their studies, the authors concluded not only that AKAP79, PKA, CaN, and membrane-associated guanylate kinase are assembled in a macromolecular complex in intact cells but also that, by FRET imaging, CaN and PKA bind to AKAP 79 within 5 nm of each other, thus extending our understanding of the level of molecular compartmentation of signaling proteins that is made possible by scaffolding proteins.	bind
27077	3	8176	6	13	NULL	NULL	NULL	AKAP79	GP		is assembled in					macromolecular complex	GP				NULL	intact cells	NULL	NULL	NULL	NULL	gw70_circulationres_94_7_866_s_115	15087426	40 From their studies, the authors concluded not only that AKAP79, PKA, CaN, and membrane-associated guanylate kinase are assembled in a macromolecular complex in intact cells but also that, by FRET imaging, CaN and PKA bind to AKAP 79 within 5 nm of each other, thus extending our understanding of the level of molecular compartmentation of signaling proteins that is made possible by scaffolding proteins.	bind
27078	4	8176	6	13	NULL	NULL	NULL	PKA	GP		is assembled in					macromolecular complex	GP				NULL	intact cells	NULL	NULL	NULL	NULL	gw70_circulationres_94_7_866_s_115	15087426	40 From their studies, the authors concluded not only that AKAP79, PKA, CaN, and membrane-associated guanylate kinase are assembled in a macromolecular complex in intact cells but also that, by FRET imaging, CaN and PKA bind to AKAP 79 within 5 nm of each other, thus extending our understanding of the level of molecular compartmentation of signaling proteins that is made possible by scaffolding proteins.	bind
27079	5	8176	6	13	NULL	NULL	NULL	CaN	GP		is assembled in					macromolecular complex	GP				NULL	intact cells	NULL	NULL	NULL	NULL	gw70_circulationres_94_7_866_s_115	15087426	40 From their studies, the authors concluded not only that AKAP79, PKA, CaN, and membrane-associated guanylate kinase are assembled in a macromolecular complex in intact cells but also that, by FRET imaging, CaN and PKA bind to AKAP 79 within 5 nm of each other, thus extending our understanding of the level of molecular compartmentation of signaling proteins that is made possible by scaffolding proteins.	bind
27080	6	8176	6	13	NULL	NULL	NULL	guanylate kinase	GP	membrane associated	is assembled in					macromolecular complex	GP				NULL	intact cells	NULL	NULL	NULL	NULL	gw70_circulationres_94_7_866_s_115	15087426	40 From their studies, the authors concluded not only that AKAP79, PKA, CaN, and membrane-associated guanylate kinase are assembled in a macromolecular complex in intact cells but also that, by FRET imaging, CaN and PKA bind to AKAP 79 within 5 nm of each other, thus extending our understanding of the level of molecular compartmentation of signaling proteins that is made possible by scaffolding proteins.	bind
32756	1	8176	7	NULL	NULL	0	NULL	AKAP79	NULL		assemble in	NULL				macromolecular complex	NULL				NULL	intact cells	0	NULL	NULL	NULL	gw70_circulationres_94_7_866_s_115	15087426	40 From their studies, the authors concluded not only that AKAP79, PKA, CaN, and membrane-associated guanylate kinase are assembled in a macromolecular complex in intact cells but also that, by FRET imaging, CaN and PKA bind to AKAP 79 within 5 nm of each other, thus extending our understanding of the level of molecular compartmentation of signaling proteins that is made possible by scaffolding proteins.	bind
32757	2	8176	7	NULL	NULL	0	NULL	PKA	NULL		assemble in	NULL				macromolecular complex	NULL				NULL	intact cells	NULL	NULL	NULL	NULL	gw70_circulationres_94_7_866_s_115	15087426	40 From their studies, the authors concluded not only that AKAP79, PKA, CaN, and membrane-associated guanylate kinase are assembled in a macromolecular complex in intact cells but also that, by FRET imaging, CaN and PKA bind to AKAP 79 within 5 nm of each other, thus extending our understanding of the level of molecular compartmentation of signaling proteins that is made possible by scaffolding proteins.	bind
32758	3	8176	7	NULL	NULL	0	NULL	CaN	NULL		assemble in	NULL				macromolecular complex	NULL				NULL	intact cells	0	NULL	NULL	NULL	gw70_circulationres_94_7_866_s_115	15087426	40 From their studies, the authors concluded not only that AKAP79, PKA, CaN, and membrane-associated guanylate kinase are assembled in a macromolecular complex in intact cells but also that, by FRET imaging, CaN and PKA bind to AKAP 79 within 5 nm of each other, thus extending our understanding of the level of molecular compartmentation of signaling proteins that is made possible by scaffolding proteins.	bind
32759	4	8176	7	10	NULL	0	NULL	guanylate kinase	NULL	membrane-associated	assemble in	NULL				macromolecular complex	NULL				NULL	intact cells	NULL	NULL	NULL	NULL	gw70_circulationres_94_7_866_s_115	15087426	40 From their studies, the authors concluded not only that AKAP79, PKA, CaN, and membrane-associated guanylate kinase are assembled in a macromolecular complex in intact cells but also that, by FRET imaging, CaN and PKA bind to AKAP 79 within 5 nm of each other, thus extending our understanding of the level of molecular compartmentation of signaling proteins that is made possible by scaffolding proteins.	bind
32760	5	8176	7	NULL	NULL	0	NULL	CaN	NULL		binds to	NULL				AKAP 79	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_7_866_s_115	15087426	40 From their studies, the authors concluded not only that AKAP79, PKA, CaN, and membrane-associated guanylate kinase are assembled in a macromolecular complex in intact cells but also that, by FRET imaging, CaN and PKA bind to AKAP 79 within 5 nm of each other, thus extending our understanding of the level of molecular compartmentation of signaling proteins that is made possible by scaffolding proteins.	bind
32761	6	8176	7	NULL	NULL	0	NULL	PKA	NULL		binds to	NULL				AKAP 79	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_7_866_s_115	15087426	40 From their studies, the authors concluded not only that AKAP79, PKA, CaN, and membrane-associated guanylate kinase are assembled in a macromolecular complex in intact cells but also that, by FRET imaging, CaN and PKA bind to AKAP 79 within 5 nm of each other, thus extending our understanding of the level of molecular compartmentation of signaling proteins that is made possible by scaffolding proteins.	bind
27081	1	8177	6	13	NULL	NULL	NULL	CaM	GP		bind					Ral	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1315_s_127	15130921	40 It has been described that binding of CaM to Ral in the presence of Ca2+ stimulates GTP binding to Ral.	bind
27082	2	8177	6	13	NULL	NULL	NULL	GTP	Chemical		bind					Ral	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1315_s_127	15130921	40 It has been described that binding of CaM to Ral in the presence of Ca2+ stimulates GTP binding to Ral.	bind
27084	3	8177	6	13	NULL	NULL	NULL	statement 1	Process		occurs in presence of					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1315_s_127	15130921	40 It has been described that binding of CaM to Ral in the presence of Ca2+ stimulates GTP binding to Ral.	bind
27085	4	8177	6	13	NULL	NULL	NULL	statement 3	Process		stimulates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1315_s_127	15130921	40 It has been described that binding of CaM to Ral in the presence of Ca2+ stimulates GTP binding to Ral.	bind
32762	1	8177	7	NULL	NULL	0	NULL	CaM	NULL		bind	NULL				Ral	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1315_s_127	15130921	40 It has been described that binding of CaM to Ral in the presence of Ca2+ stimulates GTP binding to Ral.	bind
32763	2	8177	7	NULL	NULL	0	NULL	statement 1	NULL		in presence of	NULL				Ca2+	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1315_s_127	15130921	40 It has been described that binding of CaM to Ral in the presence of Ca2+ stimulates GTP binding to Ral.	bind
32764	3	8177	7	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				Ral	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1315_s_127	15130921	40 It has been described that binding of CaM to Ral in the presence of Ca2+ stimulates GTP binding to Ral.	bind
32765	4	8177	7	NULL	NULL	0	NULL	statement 1	NULL		stimulates	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1315_s_127	15130921	40 It has been described that binding of CaM to Ral in the presence of Ca2+ stimulates GTP binding to Ral.	bind
27086	1	8181	6	13	NULL	NULL	NULL	p53	GP		bind		sequence specifically			DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_21_4462_s_420	11691934	41       Gu,W. and Roeder,R.G. (1997) Activation of p53 sequence-specific DNA binding by acetylation of the p53 C-terminal domain.	bind
27087	2	8181	6	13	NULL	NULL	NULL	statement 1	Process	activation of	occurs by					p53	GP	acetylation of	p53 C-terminal domain		NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_21_4462_s_420	11691934	41       Gu,W. and Roeder,R.G. (1997) Activation of p53 sequence-specific DNA binding by acetylation of the p53 C-terminal domain.	bind
27102	1	8182	6	13	NULL	NULL	NULL	vWF	GP		bind					collagen	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3578_s_249	9437208	41  However, HEP-PG enhanced, rather than inhibited, the binding of vWf to collagen (Fig 8  ), which is mediated also by other domains of the vWf molecule than the A1 domain, where the GP Ib- and heparin-binding areas are located.	bind
27103	2	8182	6	13	NULL	NULL	NULL	HEP-PG	GP		enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3578_s_249	9437208	41  However, HEP-PG enhanced, rather than inhibited, the binding of vWf to collagen (Fig 8  ), which is mediated also by other domains of the vWf molecule than the A1 domain, where the GP Ib- and heparin-binding areas are located.	bind
32766	1	8182	7	NULL	NULL	0	NULL	vWf	NULL		bind	NULL				collagen	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3578_s_249	9437208	41  However, HEP-PG enhanced, rather than inhibited, the binding of vWf to collagen (Fig 8  ), which is mediated also by other domains of the vWf molecule than the A1 domain, where the GP Ib- and heparin-binding areas are located.	bind
32767	2	8182	7	NULL	NULL	0	NULL	HEP-PG	NULL		enhance	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3578_s_249	9437208	41  However, HEP-PG enhanced, rather than inhibited, the binding of vWf to collagen (Fig 8  ), which is mediated also by other domains of the vWf molecule than the A1 domain, where the GP Ib- and heparin-binding areas are located.	bind
32768	3	8182	7	NULL	NULL	0	NULL	GP Ib binding site	NULL		is located in	NULL				 vWf molecule	NULL		A1 domain		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3578_s_249	9437208	41  However, HEP-PG enhanced, rather than inhibited, the binding of vWf to collagen (Fig 8  ), which is mediated also by other domains of the vWf molecule than the A1 domain, where the GP Ib- and heparin-binding areas are located.	bind
32769	4	8182	7	NULL	NULL	0	NULL	heparin-binding site	NULL		is located in	NULL				vWf molecule	NULL		A1 domain		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3578_s_249	9437208	41  However, HEP-PG enhanced, rather than inhibited, the binding of vWf to collagen (Fig 8  ), which is mediated also by other domains of the vWf molecule than the A1 domain, where the GP Ib- and heparin-binding areas are located.	bind
27104	1	8183	6	13	NULL	NULL	NULL	TnI	GP		bind		tightly			actin-Tm	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_82_2_261_s_316	9468197	41  In diastole, the actin-myosin reaction is believed to be inhibited in part by tight binding of TnI to actin-Tm.	bind
27105	2	8183	6	13	NULL	NULL	NULL	actin	GP		bind					myosin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_82_2_261_s_316	9468197	41  In diastole, the actin-myosin reaction is believed to be inhibited in part by tight binding of TnI to actin-Tm.	bind
27106	3	8183	6	13	NULL	NULL	NULL	statement 1	Process		inhibits					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_82_2_261_s_316	9468197	41  In diastole, the actin-myosin reaction is believed to be inhibited in part by tight binding of TnI to actin-Tm.	bind
32770	1	8183	7	NULL	NULL	0	NULL	TnI	NULL		bind	NULL	tightly			actin-Tm	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_82_2_261_s_316	9468197	41  In diastole, the actin-myosin reaction is believed to be inhibited in part by tight binding of TnI to actin-Tm.	bind
32771	2	8183	7	NULL	NULL	0	NULL	statement 1	NULL		inhibits	NULL				actin-myosin reaction	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_82_2_261_s_316	9468197	41  In diastole, the actin-myosin reaction is believed to be inhibited in part by tight binding of TnI to actin-Tm.	bind
27518	1	8185	6	13	NULL	NULL	NULL	serum response factors	GP		bind									CArG element of promoter	NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_3_871_s_327	10079265	41  To express alpha-SMA in response to TGF-beta1, smooth muscle cells require the binding of an undescribed factor to a TGF-beta1 control element along with the binding of serum response factors to two CArG elements in the promoter region.	bind
27519	2	8185	6	13	NULL	NULL	NULL	alpha-SMA	GP	expression of	is in response to					TGF-beta1	GP				NULL	smooth muscle cells	NULL	NULL	NULL	NULL	gw60_amjpathol_154_3_871_s_327	10079265	41  To express alpha-SMA in response to TGF-beta1, smooth muscle cells require the binding of an undescribed factor to a TGF-beta1 control element along with the binding of serum response factors to two CArG elements in the promoter region.	bind
27520	3	8185	6	13	NULL	NULL	NULL	statement 2	Process		requires					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_3_871_s_327	10079265	41  To express alpha-SMA in response to TGF-beta1, smooth muscle cells require the binding of an undescribed factor to a TGF-beta1 control element along with the binding of serum response factors to two CArG elements in the promoter region.	bind
32772	1	8185	7	NULL	NULL	0	NULL	serum response factors	NULL		bind	NULL					NULL			CArG elements	NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_3_871_s_327	10079265	41  To express alpha-SMA in response to TGF-beta1, smooth muscle cells require the binding of an undescribed factor to a TGF-beta1 control element along with the binding of serum response factors to two CArG elements in the promoter region.	bind
32773	2	8185	7	10	NULL	0	NULL	alpha-SMA 		expression of	in response to					TGF-beta1					NULL	smooth muscle cells	NULL	NULL	NULL	NULL	gw60_amjpathol_154_3_871_s_327	10079265	41  To express alpha-SMA in response to TGF-beta1, smooth muscle cells require the binding of an undescribed factor to a TGF-beta1 control element along with the binding of serum response factors to two CArG elements in the promoter region.	bind
55945	3	8185	7	10	NULL	0	NULL	statement 2			requires					statement 1					NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_3_871_s_327	10079265	41  To express alpha-SMA in response to TGF-beta1, smooth muscle cells require the binding of an undescribed factor to a TGF-beta1 control element along with the binding of serum response factors to two CArG elements in the promoter region.	bind
27107	1	8186	6	13	NULL	NULL	NULL	PG	GP		bind					EC	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_164_s_201	9012652	41  To our knowledge, we are the first to observe acute (within 15 minutes) modulation of PG binding to ECs.	bind
32774	1	8186	7	NULL	NULL	0	NULL	PG	NULL		bind	NULL				ECs	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_164_s_201	9012652	41  To our knowledge, we are the first to observe acute (within 15 minutes) modulation of PG binding to ECs.	bind
27108	1	8187	6	13	NULL	NULL	NULL	TFPI	GP		bind					factor Xa	GP		active site		NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_257	7586275	41 42  In the first step, TFPI binds to the active site of factor Xa, with formation of a TFPI - factor Xa complex with inhibited factor Xa activity.	bind
27109	2	8187	6	13	NULL	NULL	NULL	statement 1	GP		forms					TFPI - factor Xa complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_257	7586275	41 42  In the first step, TFPI binds to the active site of factor Xa, with formation of a TFPI - factor Xa complex with inhibited factor Xa activity.	bind
27110	3	8187	6	13	NULL	NULL	NULL	statement 2	Process		exhibits					factor Xa	GP	inhibited activity of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_257	7586275	41 42  In the first step, TFPI binds to the active site of factor Xa, with formation of a TFPI - factor Xa complex with inhibited factor Xa activity.	bind
32775	1	8187	7	NULL	NULL	0	NULL	TFPI	NULL		binds to	NULL				factor Xa	NULL		active site		NULL		0	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_257	7586275	41 42  In the first step, TFPI binds to the active site of factor Xa, with formation of a TFPI - factor Xa complex with inhibited factor Xa activity.	bind
32776	2	8187	7	10	NULL	0	NULL	statement 1	NULL		forms	NULL				TFPI - factor Xa complex 	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_257	7586275	41 42  In the first step, TFPI binds to the active site of factor Xa, with formation of a TFPI - factor Xa complex with inhibited factor Xa activity.	bind
32777	3	8187	7	10	NULL	0	NULL	statement 2	NULL		exhibits	NULL				factor Xa	NULL	inhibited activity of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_257	7586275	41 42  In the first step, TFPI binds to the active site of factor Xa, with formation of a TFPI - factor Xa complex with inhibited factor Xa activity.	bind
27111	1	8188	6	13	NULL	NULL	NULL	importin-alpha	GP		bind			amino acid motif		importin-beta	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_18_1031_s_161	9740803	41 amino acid motif in importin-alpha confers binding to importin-beta and hence transit into the nucleus.	bind
27112	2	8188	6	13	NULL	NULL	NULL	importin-alpha	GP		transits into					nucleus	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_18_1031_s_161	9740803	41 amino acid motif in importin-alpha confers binding to importin-beta and hence transit into the nucleus.	bind
27113	3	8188	6	13	NULL	NULL	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_18_1031_s_161	9740803	41 amino acid motif in importin-alpha confers binding to importin-beta and hence transit into the nucleus.	bind
32778	1	8188	7	NULL	NULL	0	NULL	 importin-alpha	NULL		binds to	NULL		amino acid motif		 importin-beta	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_8_18_1031_s_161	9740803	41 amino acid motif in importin-alpha confers binding to importin-beta and hence transit into the nucleus.	bind
32779	2	8188	7	NULL	NULL	0	NULL	statement 1	NULL		transit into	NULL				nucleus	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_8_18_1031_s_161	9740803	41 amino acid motif in importin-alpha confers binding to importin-beta and hence transit into the nucleus.	bind
27114	1	8189	6	13	NULL	NULL	NULL	aptamer	NucleicAcid		bind		poorly			bFGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_9_5028_s_116	12692304	41 aptamer and the control Scramble RNA bound equally poorly to bFGF ( Kd   100 nM).	bind
27115	2	8189	6	13	NULL	NULL	NULL	Scramble RNA	NucleicAcid	control	bind		poorly			bFGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_9_5028_s_116	12692304	41 aptamer and the control Scramble RNA bound equally poorly to bFGF ( Kd   100 nM).	bind
27116	3	8189	6	13	NULL	NULL	NULL	statement 1	Process	affinity of	is equal to					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_9_5028_s_116	12692304	41 aptamer and the control Scramble RNA bound equally poorly to bFGF ( Kd   100 nM).	bind
32780	1	8189	7	NULL	NULL	0	NULL	aptamer	NULL		bind	NULL	poorly			bFGF	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_100_9_5028_s_116	12692304	41 aptamer and the control Scramble RNA bound equally poorly to bFGF ( Kd   100 nM).	bind
32781	2	8189	7	10	NULL	0	NULL	Scramble RNA	NULL	control	bind	NULL	poorly			bFGF	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_9_5028_s_116	12692304	41 aptamer and the control Scramble RNA bound equally poorly to bFGF ( Kd   100 nM).	bind
55946	3	8189	7	10	NULL	0	NULL	statement 1		affinity of	is equal to					statement 2		affinity of			NULL		0	NULL	NULL	NULL	gw60_pnas_100_9_5028_s_116	12692304	41 aptamer and the control Scramble RNA bound equally poorly to bFGF ( Kd   100 nM).	bind
27117	1	8190	6	13	NULL	NULL	NULL	Grb2	GP		bind		directly			SHP-2	GP	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_81	12689916	41 Because both Grb2 65,66  and Gab1 67 can bind directly to tyrosine-phosphorylated SHP-2, it is possible that PECAM-1/SHP-2/Gab1 and PECAM-1/SHP-2/Grb2 ternary signaling complexes may form in response to certain forms of cellular stimulation.	bind
27118	2	8190	6	13	NULL	NULL	NULL	Gab1	GP		bind		directly			SHP-2	GP	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_81	12689916	41 Because both Grb2 65,66  and Gab1 67 can bind directly to tyrosine-phosphorylated SHP-2, it is possible that PECAM-1/SHP-2/Gab1 and PECAM-1/SHP-2/Grb2 ternary signaling complexes may form in response to certain forms of cellular stimulation.	bind
27521	3	8190	6	13	NULL	NULL	NULL	PECAM-1/SHP-2/Gab1 complex	GP	formation of	occurs in response to		may			cellular stimulation	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_81	12689916	41 Because both Grb2 65,66  and Gab1 67 can bind directly to tyrosine-phosphorylated SHP-2, it is possible that PECAM-1/SHP-2/Gab1 and PECAM-1/SHP-2/Grb2 ternary signaling complexes may form in response to certain forms of cellular stimulation.	bind
27522	4	8190	6	13	NULL	NULL	NULL	PECAM-1/SHP-2/Grb2 complex	GP	formation of	occurs in response to		may			cellular stimulation	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_81	12689916	41 Because both Grb2 65,66  and Gab1 67 can bind directly to tyrosine-phosphorylated SHP-2, it is possible that PECAM-1/SHP-2/Gab1 and PECAM-1/SHP-2/Grb2 ternary signaling complexes may form in response to certain forms of cellular stimulation.	bind
32782	1	8190	7	NULL	NULL	0	NULL	Grb2	NULL		bind	NULL	directly			SHP-2	NULL	phosphorylated	tyrosine		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_81	12689916	41 Because both Grb2 65,66  and Gab1 67 can bind directly to tyrosine-phosphorylated SHP-2, it is possible that PECAM-1/SHP-2/Gab1 and PECAM-1/SHP-2/Grb2 ternary signaling complexes may form in response to certain forms of cellular stimulation.	bind
32783	2	8190	7	NULL	NULL	0	NULL	Gab1	NULL		bind	NULL	directly			SHP-2	NULL	phosphorylated	tyrosine		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_81	12689916	41 Because both Grb2 65,66  and Gab1 67 can bind directly to tyrosine-phosphorylated SHP-2, it is possible that PECAM-1/SHP-2/Gab1 and PECAM-1/SHP-2/Grb2 ternary signaling complexes may form in response to certain forms of cellular stimulation.	bind
32784	3	8190	7	NULL	NULL	0	NULL	cell stimulation	NULL		form	NULL	may			PECAM-1/SHP-2/Gab1 ternary complexes	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_81	12689916	41 Because both Grb2 65,66  and Gab1 67 can bind directly to tyrosine-phosphorylated SHP-2, it is possible that PECAM-1/SHP-2/Gab1 and PECAM-1/SHP-2/Grb2 ternary signaling complexes may form in response to certain forms of cellular stimulation.	bind
32785	4	8190	7	NULL	NULL	0	NULL	cell stimulation	NULL		form	NULL	may			PECAM-1/SHP-2/Grb2 ternary signaling complexes	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_81	12689916	41 Because both Grb2 65,66  and Gab1 67 can bind directly to tyrosine-phosphorylated SHP-2, it is possible that PECAM-1/SHP-2/Gab1 and PECAM-1/SHP-2/Grb2 ternary signaling complexes may form in response to certain forms of cellular stimulation.	bind
27119	1	8191	6	13	NULL	NULL	NULL	Gab1	GP		does not bind		directly			PECAM-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_80	12689916	41 Immunoprecipitation experiments, however, were unable to demonstrate direct binding of Gab1 to PECAM-1.	bind
32997	1	8191	7	10	NULL	0	NULL	Gab1	NULL		does not bind	NULL	directly			PECAM-1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_80	12689916	41 Immunoprecipitation experiments, however, were unable to demonstrate direct binding of Gab1 to PECAM-1.	bind
27120	1	8192	6	13	NULL	NULL	NULL	IalphaI	GP		bind		weakly			serine proteinases	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1267_s_232	9777958	41 In addition, IalphaI and bikunin bind weakly with serine proteinases and consequently even at high enzyme/inhibitor ratios they have little effect on elastase and cathepsin G activity.	bind
27121	2	8192	6	13	NULL	NULL	NULL	bikunin	GP		bind		weakly			serine proteinases	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1267_s_232	9777958	41 In addition, IalphaI and bikunin bind weakly with serine proteinases and consequently even at high enzyme/inhibitor ratios they have little effect on elastase and cathepsin G activity.	bind
27122	3	8192	6	13	NULL	NULL	NULL	IalphaI	GP		has little effect on					elastase 	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1267_s_232	9777958	41 In addition, IalphaI and bikunin bind weakly with serine proteinases and consequently even at high enzyme/inhibitor ratios they have little effect on elastase and cathepsin G activity.	bind
27123	4	8192	6	13	NULL	NULL	NULL	IalphaI	GP		has little effect on					cathepsin G	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1267_s_232	9777958	41 In addition, IalphaI and bikunin bind weakly with serine proteinases and consequently even at high enzyme/inhibitor ratios they have little effect on elastase and cathepsin G activity.	bind
27124	5	8192	6	13	NULL	NULL	NULL	bikunin	GP		has little effect on					elastase	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1267_s_232	9777958	41 In addition, IalphaI and bikunin bind weakly with serine proteinases and consequently even at high enzyme/inhibitor ratios they have little effect on elastase and cathepsin G activity.	bind
27125	6	8192	6	13	NULL	NULL	NULL	bikunin	GP		has little effect on					cathepsin G	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1267_s_232	9777958	41 In addition, IalphaI and bikunin bind weakly with serine proteinases and consequently even at high enzyme/inhibitor ratios they have little effect on elastase and cathepsin G activity.	bind
32998	1	8192	7	NULL	NULL	0	NULL	IalphaI 	NULL		bind	NULL	weakly			serine proteinases	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_4_1267_s_232	9777958	41 In addition, IalphaI and bikunin bind weakly with serine proteinases and consequently even at high enzyme/inhibitor ratios they have little effect on elastase and cathepsin G activity.	bind
32999	2	8192	7	NULL	NULL	0	NULL	bikunin 	NULL		bind	NULL	weakly			serine proteinases	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_4_1267_s_232	9777958	41 In addition, IalphaI and bikunin bind weakly with serine proteinases and consequently even at high enzyme/inhibitor ratios they have little effect on elastase and cathepsin G activity.	bind
33000	3	8192	7	10	NULL	0	NULL	IalphaI	NULL		little effect on	NULL				elastase	NULL	activity of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1267_s_232	9777958	41 In addition, IalphaI and bikunin bind weakly with serine proteinases and consequently even at high enzyme/inhibitor ratios they have little effect on elastase and cathepsin G activity.	bind
33001	4	8192	7	10	NULL	0	NULL	 IalphaI 	NULL		little effect on	NULL				cathepsin G	NULL	activity of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1267_s_232	9777958	41 In addition, IalphaI and bikunin bind weakly with serine proteinases and consequently even at high enzyme/inhibitor ratios they have little effect on elastase and cathepsin G activity.	bind
33002	5	8192	7	10	NULL	0	NULL	bikunin	NULL		little effect on	NULL				elastase	NULL	activity of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1267_s_232	9777958	41 In addition, IalphaI and bikunin bind weakly with serine proteinases and consequently even at high enzyme/inhibitor ratios they have little effect on elastase and cathepsin G activity.	bind
33003	6	8192	7	10	NULL	0	NULL	bikunin	NULL		little effect on	NULL				cathepsin G	NULL	activity of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_4_1267_s_232	9777958	41 In addition, IalphaI and bikunin bind weakly with serine proteinases and consequently even at high enzyme/inhibitor ratios they have little effect on elastase and cathepsin G activity.	bind
27523	1	8193	6	13	NULL	NULL	NULL	repressor	GP	absence of;;bound	increase					PAI-1	GP	basal;; transcription of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_3_304_s_135	11804984	41 In the absence of the bound repressor, basal and stimulated PAI-1 transcription is increased.	bind
27524	2	8193	6	13	NULL	NULL	NULL	repressor	GP	absence of;;bound	increase					PAI-1	GP	stimulated;;transcription of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_3_304_s_135	11804984	41 In the absence of the bound repressor, basal and stimulated PAI-1 transcription is increased.	bind
33006	1	8193	7	10	NULL	0	NULL	repressor	NULL	absence of;;bound	increase	NULL				PAI-1	NULL	basal;; transcription of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_3_304_s_135	11804984	41 In the absence of the bound repressor, basal and stimulated PAI-1 transcription is increased.	bind
33009	2	8193	7	10	NULL	0	NULL	repressor	NULL	absence of;;bound	increase	NULL				PAI-1	NULL	stimulated;;transcription of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_3_304_s_135	11804984	41 In the absence of the bound repressor, basal and stimulated PAI-1 transcription is increased.	bind
27126	1	8194	6	13	NULL	NULL	NULL				bind			MyBP-C motif 		S2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_5_594_s_215	11909824	41, 42 Although data from the present study do not address direct or indirect effects of MyBP-C motif binding to S2, the cMyBP-C-/- knockout mice provide an ideal null background on which to test the different hypotheses because competitive effects of endogenous cMyBP-C can be excluded.	bind
33014	1	8194	7	10	NULL	0	NULL		NULL		bind	NULL		MyBP-C motif 		S2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_5_594_s_215	11909824	41, 42 Although data from the present study do not address direct or indirect effects of MyBP-C motif binding to S2, the cMyBP-C-/- knockout mice provide an ideal null background on which to test the different hypotheses because competitive effects of endogenous cMyBP-C can be excluded.	bind
27127	1	8195	6	13	NULL	NULL	NULL	PU.1	GP		bind			activation domain		RB protein	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3439_s_429	11504882	42       Hagemeier,C., Bannister,A.J., Cook,A. and Kouzarides,T. (1993) The activation domain of the transcription factor PU.1 binds the retinoblastoma (RB) protein and the transcription factor TFIID  in vitro: RB shows sequence similarity to TFIID and TFIIB.	bind
27128	2	8195	6	13	NULL	NULL	NULL	PU.1	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3439_s_429	11504882	42       Hagemeier,C., Bannister,A.J., Cook,A. and Kouzarides,T. (1993) The activation domain of the transcription factor PU.1 binds the retinoblastoma (RB) protein and the transcription factor TFIID  in vitro: RB shows sequence similarity to TFIID and TFIIB.	bind
27129	3	8195	6	13	NULL	NULL	NULL	RB	GP		is					retinoblastoma	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3439_s_429	11504882	42       Hagemeier,C., Bannister,A.J., Cook,A. and Kouzarides,T. (1993) The activation domain of the transcription factor PU.1 binds the retinoblastoma (RB) protein and the transcription factor TFIID  in vitro: RB shows sequence similarity to TFIID and TFIIB.	bind
27130	4	8195	6	13	NULL	NULL	NULL	PU.1	GP		bind			activation domain		TFIID	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3439_s_429	11504882	42       Hagemeier,C., Bannister,A.J., Cook,A. and Kouzarides,T. (1993) The activation domain of the transcription factor PU.1 binds the retinoblastoma (RB) protein and the transcription factor TFIID  in vitro: RB shows sequence similarity to TFIID and TFIIB.	bind
27131	5	8195	6	13	NULL	NULL	NULL	TFIID	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3439_s_429	11504882	42       Hagemeier,C., Bannister,A.J., Cook,A. and Kouzarides,T. (1993) The activation domain of the transcription factor PU.1 binds the retinoblastoma (RB) protein and the transcription factor TFIID  in vitro: RB shows sequence similarity to TFIID and TFIIB.	bind
27132	6	8195	6	13	NULL	NULL	NULL	RB	GP	sequence of	is similar to					TFIID	GP	sequence of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3439_s_429	11504882	42       Hagemeier,C., Bannister,A.J., Cook,A. and Kouzarides,T. (1993) The activation domain of the transcription factor PU.1 binds the retinoblastoma (RB) protein and the transcription factor TFIID  in vitro: RB shows sequence similarity to TFIID and TFIIB.	bind
27133	7	8195	6	13	NULL	NULL	NULL	RB	GP	sequence of	is similar to					TFIIB	GP	sequence of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3439_s_429	11504882	42       Hagemeier,C., Bannister,A.J., Cook,A. and Kouzarides,T. (1993) The activation domain of the transcription factor PU.1 binds the retinoblastoma (RB) protein and the transcription factor TFIID  in vitro: RB shows sequence similarity to TFIID and TFIIB.	bind
33019	1	8195	7	NULL	NULL	0	NULL	PU.1	NULL		binds	NULL		activation domain		RB protein	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3439_s_429	11504882	42       Hagemeier,C., Bannister,A.J., Cook,A. and Kouzarides,T. (1993) The activation domain of the transcription factor PU.1 binds the retinoblastoma (RB) protein and the transcription factor TFIID  in vitro: RB shows sequence similarity to TFIID and TFIIB.	bind
33020	2	8195	7	NULL	NULL	0	NULL	PU.1	NULL		binds	NULL		activation domain		TFIID	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3439_s_429	11504882	42       Hagemeier,C., Bannister,A.J., Cook,A. and Kouzarides,T. (1993) The activation domain of the transcription factor PU.1 binds the retinoblastoma (RB) protein and the transcription factor TFIID  in vitro: RB shows sequence similarity to TFIID and TFIIB.	bind
33022	3	8195	7	NULL	NULL	0	NULL	PU.1	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3439_s_429	11504882	42       Hagemeier,C., Bannister,A.J., Cook,A. and Kouzarides,T. (1993) The activation domain of the transcription factor PU.1 binds the retinoblastoma (RB) protein and the transcription factor TFIID  in vitro: RB shows sequence similarity to TFIID and TFIIB.	bind
33023	4	8195	7	NULL	NULL	0	NULL	TFIID	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3439_s_429	11504882	42       Hagemeier,C., Bannister,A.J., Cook,A. and Kouzarides,T. (1993) The activation domain of the transcription factor PU.1 binds the retinoblastoma (RB) protein and the transcription factor TFIID  in vitro: RB shows sequence similarity to TFIID and TFIIB.	bind
33024	5	8195	7	NULL	NULL	0	NULL	RB	NULL	Sequence of	is similar to	NULL				TFIID	NULL	sequence of			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3439_s_429	11504882	42       Hagemeier,C., Bannister,A.J., Cook,A. and Kouzarides,T. (1993) The activation domain of the transcription factor PU.1 binds the retinoblastoma (RB) protein and the transcription factor TFIID  in vitro: RB shows sequence similarity to TFIID and TFIIB.	bind
33025	6	8195	7	NULL	NULL	0	NULL	RB	NULL	sequence of	is similar to	NULL				TFIIB	NULL	sequence of			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3439_s_429	11504882	42       Hagemeier,C., Bannister,A.J., Cook,A. and Kouzarides,T. (1993) The activation domain of the transcription factor PU.1 binds the retinoblastoma (RB) protein and the transcription factor TFIID  in vitro: RB shows sequence similarity to TFIID and TFIIB.	bind
46606	7	8195	7	10	NULL	0	NULL	RB	NULL		is	NULL				retinoblastoma	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3439_s_429	11504882	42       Hagemeier,C., Bannister,A.J., Cook,A. and Kouzarides,T. (1993) The activation domain of the transcription factor PU.1 binds the retinoblastoma (RB) protein and the transcription factor TFIID  in vitro: RB shows sequence similarity to TFIID and TFIIB.	bind
27525	1	8196	6	13	NULL	NULL	NULL	U1A	GP		is a type of					spliceosomal protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_550_s_390	11788718	42       Rimmele,M. and Belasco,J. (1998) Target discrimination by RNA-binding proteins: role of the ancillary protein U2A'' and a critical leucine residue in differentiating the RNA-binding specificity of spliceosomal proteins U1A and U2B'''.	bind
27526	2	8196	6	13	NULL	NULL	NULL	U2B'''	GP		is a type of					splicosomal protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_550_s_390	11788718	42       Rimmele,M. and Belasco,J. (1998) Target discrimination by RNA-binding proteins: role of the ancillary protein U2A'' and a critical leucine residue in differentiating the RNA-binding specificity of spliceosomal proteins U1A and U2B'''.	bind
27527	3	8196	6	13	NULL	NULL	NULL	U2A"	GP		is a type of					ancillary protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_550_s_390	11788718	42       Rimmele,M. and Belasco,J. (1998) Target discrimination by RNA-binding proteins: role of the ancillary protein U2A'' and a critical leucine residue in differentiating the RNA-binding specificity of spliceosomal proteins U1A and U2B'''.	bind
27528	4	8196	6	13	NULL	NULL	NULL	U1A	GP		bind					RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_550_s_390	11788718	42       Rimmele,M. and Belasco,J. (1998) Target discrimination by RNA-binding proteins: role of the ancillary protein U2A'' and a critical leucine residue in differentiating the RNA-binding specificity of spliceosomal proteins U1A and U2B'''.	bind
27529	5	8196	6	13	NULL	NULL	NULL	U2B"'	GP		bind					RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_550_s_390	11788718	42       Rimmele,M. and Belasco,J. (1998) Target discrimination by RNA-binding proteins: role of the ancillary protein U2A'' and a critical leucine residue in differentiating the RNA-binding specificity of spliceosomal proteins U1A and U2B'''.	bind
33026	1	8196	7	NULL	NULL	0	NULL	U1A 	NULL		bind	NULL				RNA	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_550_s_390	11788718	42       Rimmele,M. and Belasco,J. (1998) Target discrimination by RNA-binding proteins: role of the ancillary protein U2A'' and a critical leucine residue in differentiating the RNA-binding specificity of spliceosomal proteins U1A and U2B'''.	bind
33027	2	8196	7	10	NULL	0	NULL	U2B"'	NULL		bind	NULL				RNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_550_s_390	11788718	42       Rimmele,M. and Belasco,J. (1998) Target discrimination by RNA-binding proteins: role of the ancillary protein U2A'' and a critical leucine residue in differentiating the RNA-binding specificity of spliceosomal proteins U1A and U2B'''.	bind
33028	3	8196	7	NULL	NULL	0	NULL	U1A	NULL		is a type of	NULL				spliceosomal proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_550_s_390	11788718	42       Rimmele,M. and Belasco,J. (1998) Target discrimination by RNA-binding proteins: role of the ancillary protein U2A'' and a critical leucine residue in differentiating the RNA-binding specificity of spliceosomal proteins U1A and U2B'''.	bind
33029	4	8196	7	10	NULL	0	NULL	U2B"'	NULL		is a type of	NULL				spliceosomal proteins	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_550_s_390	11788718	42       Rimmele,M. and Belasco,J. (1998) Target discrimination by RNA-binding proteins: role of the ancillary protein U2A'' and a critical leucine residue in differentiating the RNA-binding specificity of spliceosomal proteins U1A and U2B'''.	bind
46607	5	8196	7	10	NULL	0	NULL	U2A''	NULL		is a type of	NULL				ancillary protein	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_550_s_390	11788718	42       Rimmele,M. and Belasco,J. (1998) Target discrimination by RNA-binding proteins: role of the ancillary protein U2A'' and a critical leucine residue in differentiating the RNA-binding specificity of spliceosomal proteins U1A and U2B'''.	bind
33030	1	8197	7	13	NULL	NULL	NULL	protein	GP	mutant	bind					HDL	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_1_210_s_176	10634820	42  Although replacement of various amino acids in the  C-terminus demonstrated that substitution of specifically charged residues between 195 and 238 did not affect the binding of mutant protein to HDL, 16  penetration of exchangeable apolipoproteins in the phospholipid layer involves both electrostatic and hydrophobic interactions.	bind
33031	2	8197	7	NULL	NULL	0	NULL		NULL		substituted with	NULL		C-terminus aminoacid			NULL		charged residues between 195 and 238		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_1_210_s_176	10634820	42  Although replacement of various amino acids in the  C-terminus demonstrated that substitution of specifically charged residues between 195 and 238 did not affect the binding of mutant protein to HDL, 16  penetration of exchangeable apolipoproteins in the phospholipid layer involves both electrostatic and hydrophobic interactions.	bind
33032	3	8197	7	13	NULL	NULL	NULL	statement 2	Process		does not affect					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_1_210_s_176	10634820	42  Although replacement of various amino acids in the  C-terminus demonstrated that substitution of specifically charged residues between 195 and 238 did not affect the binding of mutant protein to HDL, 16  penetration of exchangeable apolipoproteins in the phospholipid layer involves both electrostatic and hydrophobic interactions.	bind
33033	4	8197	7	13	NULL	NULL	NULL	apolipoproteins	GP	penetration of	involves					electrostatic interactions	Process				NULL	phospholipid layer	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_1_210_s_176	10634820	42  Although replacement of various amino acids in the  C-terminus demonstrated that substitution of specifically charged residues between 195 and 238 did not affect the binding of mutant protein to HDL, 16  penetration of exchangeable apolipoproteins in the phospholipid layer involves both electrostatic and hydrophobic interactions.	bind
33034	5	8197	7	13	NULL	NULL	NULL	apolipoproteins	GP	penetration of	involves					hydrophobic interactions	Process				NULL	phospholipid layer	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_1_210_s_176	10634820	42  Although replacement of various amino acids in the  C-terminus demonstrated that substitution of specifically charged residues between 195 and 238 did not affect the binding of mutant protein to HDL, 16  penetration of exchangeable apolipoproteins in the phospholipid layer involves both electrostatic and hydrophobic interactions.	bind
27134	1	8198	6	13	NULL	NULL	NULL	FKBP12.6	GP		bind					FK506	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_6_990_s_31	8635249	42  FKBP12.6 binds FK506 and rapamycin and is a candidate for the form associated with the cardiac RyR.	bind
27135	2	8198	6	13	NULL	NULL	NULL	FKBP12.6	GP		bind					rapamycin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_6_990_s_31	8635249	42  FKBP12.6 binds FK506 and rapamycin and is a candidate for the form associated with the cardiac RyR.	bind
27136	3	8198	6	13	NULL	NULL	NULL	FKBP12.6	GP		is associated with					RyR 	GP	cardiac			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_6_990_s_31	8635249	42  FKBP12.6 binds FK506 and rapamycin and is a candidate for the form associated with the cardiac RyR.	bind
33035	1	8198	7	NULL	NULL	0	NULL	FKBP12.6	NULL		binds	NULL				FK506	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_78_6_990_s_31	8635249	42  FKBP12.6 binds FK506 and rapamycin and is a candidate for the form associated with the cardiac RyR.	bind
33036	2	8198	7	NULL	NULL	0	NULL	FKBP12.6	NULL		binds	NULL				rapamycin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_78_6_990_s_31	8635249	42  FKBP12.6 binds FK506 and rapamycin and is a candidate for the form associated with the cardiac RyR.	bind
33037	3	8198	7	10	NULL	0	NULL	FKBP12.6	NULL		is associated with	NULL				RyR	NULL	cardiac			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_6_990_s_31	8635249	42  FKBP12.6 binds FK506 and rapamycin and is a candidate for the form associated with the cardiac RyR.	bind
27137	2	8199	6	13	NULL	NULL	NULL	Egr-1	GP		bind					SRR-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3406_s_244	9437186	42  Further studies are needed to show whether the suppression of Egr-1 binding to SRR-2 in cells treated with curcumin is the result of inhibition of de novo synthesis of Egr-1 or the diminished phosphorylation of Egr-1.	bind
27138	4	8199	6	13	NULL	NULL	NULL	statement 2	Process		suppressed in					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3406_s_244	9437186	42  Further studies are needed to show whether the suppression of Egr-1 binding to SRR-2 in cells treated with curcumin is the result of inhibition of de novo synthesis of Egr-1 or the diminished phosphorylation of Egr-1.	bind
46608	1	8199	6	13	NULL	NULL	NULL	cells	Cell		is treated with					curcumin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3406_s_244	9437186	42  Further studies are needed to show whether the suppression of Egr-1 binding to SRR-2 in cells treated with curcumin is the result of inhibition of de novo synthesis of Egr-1 or the diminished phosphorylation of Egr-1.	bind
46609	3	8199	6	13	NULL	NULL	NULL	statement 2	Process		occurs in					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3406_s_244	9437186	42  Further studies are needed to show whether the suppression of Egr-1 binding to SRR-2 in cells treated with curcumin is the result of inhibition of de novo synthesis of Egr-1 or the diminished phosphorylation of Egr-1.	bind
33038	2	8199	7	10	NULL	0	NULL	Egr-1	NULL		bind	NULL				SRR-2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3406_s_244	9437186	42  Further studies are needed to show whether the suppression of Egr-1 binding to SRR-2 in cells treated with curcumin is the result of inhibition of de novo synthesis of Egr-1 or the diminished phosphorylation of Egr-1.	bind
46610	1	8199	7	10	NULL	0	NULL	cells	NULL		is treated with	NULL				curcumin	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3406_s_244	9437186	42  Further studies are needed to show whether the suppression of Egr-1 binding to SRR-2 in cells treated with curcumin is the result of inhibition of de novo synthesis of Egr-1 or the diminished phosphorylation of Egr-1.	bind
46611	3	8199	7	10	NULL	0	NULL	statement 2	NULL		occurs in	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3406_s_244	9437186	42  Further studies are needed to show whether the suppression of Egr-1 binding to SRR-2 in cells treated with curcumin is the result of inhibition of de novo synthesis of Egr-1 or the diminished phosphorylation of Egr-1.	bind
46612	4	8199	7	10	NULL	0	NULL	statement 2	NULL		suppressed in	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3406_s_244	9437186	42  Further studies are needed to show whether the suppression of Egr-1 binding to SRR-2 in cells treated with curcumin is the result of inhibition of de novo synthesis of Egr-1 or the diminished phosphorylation of Egr-1.	bind
27139	1	8200	6	13	NULL	NULL	NULL	TGF-betaR:Fc	GP		does not bind					TGF-beta2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_10_1212_s_232	10347096	42  Similarly, TGF-betaR:Fc used here did not bind TGF-beta2 in an ELISA (data not shown), which is consistent with the notion that this isoform requires presentation by betaglycan for binding to the TGF-betaRII.	bind
27154	2	8200	6	13	NULL	NULL	NULL	TGF-betaR:Fc	GP		bind					TGF-betaRII	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_10_1212_s_232	10347096	42  Similarly, TGF-betaR:Fc used here did not bind TGF-beta2 in an ELISA (data not shown), which is consistent with the notion that this isoform requires presentation by betaglycan for binding to the TGF-betaRII.	bind
27156	3	8200	6	13	NULL	NULL	NULL	statement 2	Process		requires					betaglycan	GP	presentation by 			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_10_1212_s_232	10347096	42  Similarly, TGF-betaR:Fc used here did not bind TGF-beta2 in an ELISA (data not shown), which is consistent with the notion that this isoform requires presentation by betaglycan for binding to the TGF-betaRII.	bind
33039	1	8200	7	NULL	NULL	0	NULL	TGF-betaR:Fc	NULL		does not bind	NULL				TGF-beta2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_10_1212_s_232	10347096	42  Similarly, TGF-betaR:Fc used here did not bind TGF-beta2 in an ELISA (data not shown), which is consistent with the notion that this isoform requires presentation by betaglycan for binding to the TGF-betaRII.	bind
33040	2	8200	7	NULL	NULL	0	NULL	TGF-betaR:Fc	NULL		bind	NULL				TGF-betaRII	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_10_1212_s_232	10347096	42  Similarly, TGF-betaR:Fc used here did not bind TGF-beta2 in an ELISA (data not shown), which is consistent with the notion that this isoform requires presentation by betaglycan for binding to the TGF-betaRII.	bind
33041	3	8200	7	NULL	NULL	0	NULL	statement 2	NULL		requires	NULL				betaglycan	NULL	presentation by 			NULL		0	NULL	NULL	NULL	gw60_circulationres_84_10_1212_s_232	10347096	42  Similarly, TGF-betaR:Fc used here did not bind TGF-beta2 in an ELISA (data not shown), which is consistent with the notion that this isoform requires presentation by betaglycan for binding to the TGF-betaRII.	bind
27158	1	8201	6	13	NULL	NULL	NULL	vWF	GP		bind					collagen	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3578_s_250	9437208	42  The enhanced binding of vWf to collagen may have sealed the platelet-activating domains of collagen.	bind
27162	2	8201	6	13	NULL	NULL	NULL	statement 1	Process		seal		may			collagen	GP		platelet-activating domain		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3578_s_250	9437208	42  The enhanced binding of vWf to collagen may have sealed the platelet-activating domains of collagen.	bind
33042	1	8201	7	NULL	NULL	0	NULL	vWf	NULL		bind	NULL				collagen	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3578_s_250	9437208	42  The enhanced binding of vWf to collagen may have sealed the platelet-activating domains of collagen.	bind
33043	2	8201	7	10	NULL	0	NULL	statement 1	NULL		seal	NULL	may			collagen	NULL		 platelet-activating domains		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3578_s_250	9437208	42  The enhanced binding of vWf to collagen may have sealed the platelet-activating domains of collagen.	bind
27163	1	8202	6	13	NULL	NULL	NULL	BKLF/TEF-2	GP		bind		strongly							CACC box	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_2_182_s_265	10417400	42 43  The BKLF/TEF-2, another member of Kruppel family of transcription factors, which binds strongly to CACC box, contains a unique basic region and its expression is less tissue restricted.	bind
27164	2	8202	6	13	NULL	NULL	NULL	BKLF/TEF-2	GP		is a member of					Kruppel family of transcription factors	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_2_182_s_265	10417400	42 43  The BKLF/TEF-2, another member of Kruppel family of transcription factors, which binds strongly to CACC box, contains a unique basic region and its expression is less tissue restricted.	bind
27165	3	8202	6	13	NULL	NULL	NULL	BKLF/TEF-2	GP		contains a							unique	basic region		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_2_182_s_265	10417400	42 43  The BKLF/TEF-2, another member of Kruppel family of transcription factors, which binds strongly to CACC box, contains a unique basic region and its expression is less tissue restricted.	bind
27166	4	8202	6	13	NULL	NULL	NULL	BKLF/TEF-2	GP	expression of	is					tissue restricted		less			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_2_182_s_265	10417400	42 43  The BKLF/TEF-2, another member of Kruppel family of transcription factors, which binds strongly to CACC box, contains a unique basic region and its expression is less tissue restricted.	bind
33044	1	8202	7	NULL	NULL	0	NULL	BKLF/TEF-2	NULL		binds	NULL	strongly				NULL			CACC box	NULL		0	NULL	NULL	NULL	gw60_circulationres_85_2_182_s_265	10417400	42 43  The BKLF/TEF-2, another member of Kruppel family of transcription factors, which binds strongly to CACC box, contains a unique basic region and its expression is less tissue restricted.	bind
33045	2	8202	7	10	NULL	0	NULL	BKLF/TEF-2	NULL		is a member of	NULL				Kruppel family of transcription factors	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_2_182_s_265	10417400	42 43  The BKLF/TEF-2, another member of Kruppel family of transcription factors, which binds strongly to CACC box, contains a unique basic region and its expression is less tissue restricted.	bind
33046	3	8202	7	10	NULL	0	NULL		NULL		contains	NULL			CACC box	basic region	NULL	unique			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_2_182_s_265	10417400	42 43  The BKLF/TEF-2, another member of Kruppel family of transcription factors, which binds strongly to CACC box, contains a unique basic region and its expression is less tissue restricted.	bind
33047	4	8202	7	NULL	NULL	0	NULL		NULL	expression of	is less 	NULL			CACC box	tissue restricted	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_85_2_182_s_265	10417400	42 43  The BKLF/TEF-2, another member of Kruppel family of transcription factors, which binds strongly to CACC box, contains a unique basic region and its expression is less tissue restricted.	bind
27167	1	8203	6	13	NULL	NULL	NULL	apoA-I	GP		bind		directly			ABCA1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_74	12738681	42 Because apoA-I directly binds ABCA1, we speculated that apoA-I might regulate ABCA1 protein turnover.	bind
27168	2	8203	6	13	NULL	NULL	NULL	apo A-I	GP		regulate		might			ABCA1 protein	GP	turnover of 			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_74	12738681	42 Because apoA-I directly binds ABCA1, we speculated that apoA-I might regulate ABCA1 protein turnover.	bind
33090	1	8203	7	NULL	NULL	0	NULL	apoA-I	NULL		binds	NULL	directly			ABCA1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_74	12738681	42 Because apoA-I directly binds ABCA1, we speculated that apoA-I might regulate ABCA1 protein turnover.	bind
33091	2	8203	7	10	NULL	0	NULL	apoA-I	NULL		regulate	NULL	might			ABCA1 protein	NULL	turnover of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_74	12738681	42 Because apoA-I directly binds ABCA1, we speculated that apoA-I might regulate ABCA1 protein turnover.	bind
27169	1	8204	6	13	NULL	NULL	NULL	E7	GP		bind					p130/Rb	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_5_1623_s_237	11073822	42 In contrast to Rb, however, binding of E7 to p130/Rb does not lead to increase proteolytic degradation.	bind
27170	2	8204	6	13	NULL	NULL	NULL	statement 1	Process		does not increase					proteolytic degradation	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_5_1623_s_237	11073822	42 In contrast to Rb, however, binding of E7 to p130/Rb does not lead to increase proteolytic degradation.	bind
33092	1	8204	7	NULL	NULL	0	NULL	E7 	NULL		bind	NULL				p130/Rb	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_5_1623_s_237	11073822	42 In contrast to Rb, however, binding of E7 to p130/Rb does not lead to increase proteolytic degradation.	bind
33093	2	8204	7	NULL	NULL	0	NULL	statement 1	NULL		does not increase	NULL				proteolytic degradation	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_5_1623_s_237	11073822	42 In contrast to Rb, however, binding of E7 to p130/Rb does not lead to increase proteolytic degradation.	bind
33094	3	8204	7	NULL	NULL	0	NULL	E7	NULL		bind	NULL				Rb	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_5_1623_s_237	11073822	42 In contrast to Rb, however, binding of E7 to p130/Rb does not lead to increase proteolytic degradation.	bind
27171	1	8205	6	13	NULL	NULL	NULL	MMP gene	GP		bind				AP-1 element of promoter	members of the AP-1 transcription factor family	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1353_s_112	15860743	42 Interestingly, a single AP-1 element, which binds members of the AP-1 transcription factor family, is found in the promoter region of each inducible MMP gene.	bind
33095	1	8205	7	NULL	NULL	0	NULL		NULL		binds	NULL			AP-1 element	AP-1 transcription factor family	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1353_s_112	15860743	42 Interestingly, a single AP-1 element, which binds members of the AP-1 transcription factor family, is found in the promoter region of each inducible MMP gene.	bind
33096	2	8205	7	10	NULL	0	NULL				is found in				AP-1 element	MMP gene				promoter	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_7_1353_s_112	15860743	42 Interestingly, a single AP-1 element, which binds members of the AP-1 transcription factor family, is found in the promoter region of each inducible MMP gene.	bind
27530	1	8206	6	13	NULL	NULL	NULL	Ral GEF	GP		is			PH domain;; SH3 binding motif		RalGPS	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1315_s_132	15130921	42 This RalGPS (Ral GEFs with  PH domain and  SH3 binding motif) or RalGEF2 was unable to bind to and induce nucleotide exchange of a C-terminally truncated Ral mutant, suggesting that the C-terminus of Ral is required for RalGEF2 binding.	bind
27531	2	8206	6	13	NULL	NULL	NULL	RalGEF2	GP		does not bind					Ral	GP	truncated;;mutant	C-terminus		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1315_s_132	15130921	42 This RalGPS (Ral GEFs with  PH domain and  SH3 binding motif) or RalGEF2 was unable to bind to and induce nucleotide exchange of a C-terminally truncated Ral mutant, suggesting that the C-terminus of Ral is required for RalGEF2 binding.	bind
27532	3	8206	6	13	NULL	NULL	NULL	RalGEF2	GP		does not induce					Ral	GP	nucleotide exchange of;; mutant;; truncated	C-terminal		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1315_s_132	15130921	42 This RalGPS (Ral GEFs with  PH domain and  SH3 binding motif) or RalGEF2 was unable to bind to and induce nucleotide exchange of a C-terminally truncated Ral mutant, suggesting that the C-terminus of Ral is required for RalGEF2 binding.	bind
27533	4	8206	6	13	NULL	NULL	NULL	Ral	GP		is required for			C-terminus		RalGEF2	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1315_s_132	15130921	42 This RalGPS (Ral GEFs with  PH domain and  SH3 binding motif) or RalGEF2 was unable to bind to and induce nucleotide exchange of a C-terminally truncated Ral mutant, suggesting that the C-terminus of Ral is required for RalGEF2 binding.	bind
33097	1	8206	7	10	NULL	0	NULL	Ral	NULL	truncated;;mutant	exchange	NULL		C-terminal		nucleotide	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1315_s_132	15130921	42 This RalGPS (Ral GEFs with  PH domain and  SH3 binding motif) or RalGEF2 was unable to bind to and induce nucleotide exchange of a C-terminally truncated Ral mutant, suggesting that the C-terminus of Ral is required for RalGEF2 binding.	bind
33098	2	8206	7	NULL	NULL	0	NULL	RalGEF2	NULL		does not bind	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1315_s_132	15130921	42 This RalGPS (Ral GEFs with  PH domain and  SH3 binding motif) or RalGEF2 was unable to bind to and induce nucleotide exchange of a C-terminally truncated Ral mutant, suggesting that the C-terminus of Ral is required for RalGEF2 binding.	bind
33099	3	8206	7	NULL	NULL	0	NULL	RalGEF2	NULL		does not induce	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1315_s_132	15130921	42 This RalGPS (Ral GEFs with  PH domain and  SH3 binding motif) or RalGEF2 was unable to bind to and induce nucleotide exchange of a C-terminally truncated Ral mutant, suggesting that the C-terminus of Ral is required for RalGEF2 binding.	bind
33100	4	8206	7	NULL	NULL	0	NULL	RalGPS	NULL		does not bind	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1315_s_132	15130921	42 This RalGPS (Ral GEFs with  PH domain and  SH3 binding motif) or RalGEF2 was unable to bind to and induce nucleotide exchange of a C-terminally truncated Ral mutant, suggesting that the C-terminus of Ral is required for RalGEF2 binding.	bind
33101	5	8206	7	NULL	NULL	0	NULL	RalGPS	NULL		does not induce	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1315_s_132	15130921	42 This RalGPS (Ral GEFs with  PH domain and  SH3 binding motif) or RalGEF2 was unable to bind to and induce nucleotide exchange of a C-terminally truncated Ral mutant, suggesting that the C-terminus of Ral is required for RalGEF2 binding.	bind
33102	6	8206	7	10	NULL	0	NULL	RalGPS	NULL		consist of	NULL				Ral GEFs	NULL		PH domain;;SH3 binding motif		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1315_s_132	15130921	42 This RalGPS (Ral GEFs with  PH domain and  SH3 binding motif) or RalGEF2 was unable to bind to and induce nucleotide exchange of a C-terminally truncated Ral mutant, suggesting that the C-terminus of Ral is required for RalGEF2 binding.	bind
33103	7	8206	7	NULL	NULL	0	NULL	Ral	NULL		is required for	NULL		C-terminus		RalGEF2	NULL	binding of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_7_1315_s_132	15130921	42 This RalGPS (Ral GEFs with  PH domain and  SH3 binding motif) or RalGEF2 was unable to bind to and induce nucleotide exchange of a C-terminally truncated Ral mutant, suggesting that the C-terminus of Ral is required for RalGEF2 binding.	bind
27181	1	8208	6	13	NULL	NULL	NULL	uPAR	GP		bind					CD11b/CD18	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_163_2_517_s_275	12875972	42-44  This receptor is involved in cellular movement by generating cell-surface Pm activity, via uPA binding, and by uPAR binding to beta2-integrins, particularly CD11b/CD18 (Mac-1).	bind
27182	2	8208	6	13	NULL	NULL	NULL	CD11b/CD18	GP		is a type of					beta2-integrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_163_2_517_s_275	12875972	42-44  This receptor is involved in cellular movement by generating cell-surface Pm activity, via uPA binding, and by uPAR binding to beta2-integrins, particularly CD11b/CD18 (Mac-1).	bind
55947	3	8208	6	13	NULL	NULL	NULL	CD11b/CD18	GP		is					Mac-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_163_2_517_s_275	12875972	42-44  This receptor is involved in cellular movement by generating cell-surface Pm activity, via uPA binding, and by uPAR binding to beta2-integrins, particularly CD11b/CD18 (Mac-1).	bind
33106	2	8208	7	NULL	NULL	0	NULL	uPAR	NULL		bind	NULL				CD11b/CD18	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_163_2_517_s_275	12875972	42-44  This receptor is involved in cellular movement by generating cell-surface Pm activity, via uPA binding, and by uPAR binding to beta2-integrins, particularly CD11b/CD18 (Mac-1).	bind
33107	3	8208	7	NULL	NULL	0	NULL	CD11b/CD18	NULL		is	NULL				Mac-1	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_163_2_517_s_275	12875972	42-44  This receptor is involved in cellular movement by generating cell-surface Pm activity, via uPA binding, and by uPAR binding to beta2-integrins, particularly CD11b/CD18 (Mac-1).	bind
33108	4	8208	7	NULL	NULL	0	NULL	CD11b/CD18	NULL		is a type of	NULL				beta2-integrins	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_163_2_517_s_275	12875972	42-44  This receptor is involved in cellular movement by generating cell-surface Pm activity, via uPA binding, and by uPAR binding to beta2-integrins, particularly CD11b/CD18 (Mac-1).	bind
27183	1	8209	6	13	NULL	NULL	NULL	type II nuclear receptors	GP		bind									full site estrogen response element	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_366	11452016	43       Klinge,C.M., Bodenner,D.L., Desai,D., Niles,R.M. and Traish,A.M. (1997) Binding of type II nuclear receptors and estrogen receptor to full and half-site estrogen response elements  in vitro.	bind
27184	2	8209	6	13	NULL	NULL	NULL	type II nuclear receptors	GP		bind									half-site estrogen response element	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_366	11452016	43       Klinge,C.M., Bodenner,D.L., Desai,D., Niles,R.M. and Traish,A.M. (1997) Binding of type II nuclear receptors and estrogen receptor to full and half-site estrogen response elements  in vitro.	bind
27185	3	8209	6	13	NULL	NULL	NULL	estrogen receptor	GP		bind									full site estrogen response element	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_366	11452016	43       Klinge,C.M., Bodenner,D.L., Desai,D., Niles,R.M. and Traish,A.M. (1997) Binding of type II nuclear receptors and estrogen receptor to full and half-site estrogen response elements  in vitro.	bind
27186	4	8209	6	13	NULL	NULL	NULL	estrogen receptor	GP		bind									half-site estrogen response element	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_366	11452016	43       Klinge,C.M., Bodenner,D.L., Desai,D., Niles,R.M. and Traish,A.M. (1997) Binding of type II nuclear receptors and estrogen receptor to full and half-site estrogen response elements  in vitro.	bind
33109	1	8209	7	NULL	NULL	0	NULL	type II nuclear receptors 	NULL		binds to	NULL					NULL			full-site estrogen response element	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_366	11452016	43       Klinge,C.M., Bodenner,D.L., Desai,D., Niles,R.M. and Traish,A.M. (1997) Binding of type II nuclear receptors and estrogen receptor to full and half-site estrogen response elements  in vitro.	bind
33110	2	8209	7	NULL	NULL	0	NULL	estrogen receptor	NULL		binds to	NULL					NULL			full-site estrogen response element	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_366	11452016	43       Klinge,C.M., Bodenner,D.L., Desai,D., Niles,R.M. and Traish,A.M. (1997) Binding of type II nuclear receptors and estrogen receptor to full and half-site estrogen response elements  in vitro.	bind
47494	3	8209	7	NULL	NULL	0	NULL	type II nuclear receptors	NULL		bind	NULL					NULL			half-site estrogen response element	NULL	in vitro	0	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_366	11452016	43       Klinge,C.M., Bodenner,D.L., Desai,D., Niles,R.M. and Traish,A.M. (1997) Binding of type II nuclear receptors and estrogen receptor to full and half-site estrogen response elements  in vitro.	bind
47495	4	8209	7	NULL	NULL	0	NULL	estrogen receptor	NULL		bind	NULL					NULL			half-site estrogen response element	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_366	11452016	43       Klinge,C.M., Bodenner,D.L., Desai,D., Niles,R.M. and Traish,A.M. (1997) Binding of type II nuclear receptors and estrogen receptor to full and half-site estrogen response elements  in vitro.	bind
27187	1	8210	6	13	NULL	NULL	NULL	RNA	NucleicAcid		bind		sequence specifically			Nova	GP		KH domain		NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_638_s_301	11160884	43       Lewis,H.A., Musunuru,K., Jensen,K.B., Edo,C., Chen,H., Darnell,R.B. and Burley,S.K. (2000) Sequence-specific RNA binding by a Nova KH domain: implications for paraneoplastic disease and the fragile X syndrome.	bind
27188	2	8210	6	13	NULL	NULL	NULL	statement 1	Process		implies for					paraneoplastic disease	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_638_s_301	11160884	43       Lewis,H.A., Musunuru,K., Jensen,K.B., Edo,C., Chen,H., Darnell,R.B. and Burley,S.K. (2000) Sequence-specific RNA binding by a Nova KH domain: implications for paraneoplastic disease and the fragile X syndrome.	bind
27189	3	8210	6	13	NULL	NULL	NULL	statement 1	Process		implies for					fragile X syndrome	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_638_s_301	11160884	43       Lewis,H.A., Musunuru,K., Jensen,K.B., Edo,C., Chen,H., Darnell,R.B. and Burley,S.K. (2000) Sequence-specific RNA binding by a Nova KH domain: implications for paraneoplastic disease and the fragile X syndrome.	bind
33111	1	8210	7	10	NULL	0	NULL	Nova	NULL		bind	NULL	sequence-specific	KH domain		RNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_638_s_301	11160884	43       Lewis,H.A., Musunuru,K., Jensen,K.B., Edo,C., Chen,H., Darnell,R.B. and Burley,S.K. (2000) Sequence-specific RNA binding by a Nova KH domain: implications for paraneoplastic disease and the fragile X syndrome.	bind
33112	2	8210	7	NULL	NULL	0	NULL	statement 1	NULL		implicates	NULL				paraneoplastic disease	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_638_s_301	11160884	43       Lewis,H.A., Musunuru,K., Jensen,K.B., Edo,C., Chen,H., Darnell,R.B. and Burley,S.K. (2000) Sequence-specific RNA binding by a Nova KH domain: implications for paraneoplastic disease and the fragile X syndrome.	bind
33114	3	8210	7	NULL	NULL	0	NULL	statement 1	NULL		implicates	NULL				fragile X syndrome	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_638_s_301	11160884	43       Lewis,H.A., Musunuru,K., Jensen,K.B., Edo,C., Chen,H., Darnell,R.B. and Burley,S.K. (2000) Sequence-specific RNA binding by a Nova KH domain: implications for paraneoplastic disease and the fragile X syndrome.	bind
27190	1	8211	6	13	NULL	NULL	NULL	2C4 monoclonal mouse-antirabbit antibody	GP		bind					class II MHC antigen	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2515_s_81	9409222	43  As a marker of inflammation with activation of the immune system, the 2C4 monoclonal mouse-antirabbit antibody (Serotec, Oxford, England), which binds to the rabbit homologue of the class II major histocompatibility complex (MHC) antigen, was used in cryostat sections of aortic allografts.	bind
27191	2	8211	6	13	NULL	NULL	NULL	MHC	GP		is					major histocompatibility complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2515_s_81	9409222	43  As a marker of inflammation with activation of the immune system, the 2C4 monoclonal mouse-antirabbit antibody (Serotec, Oxford, England), which binds to the rabbit homologue of the class II major histocompatibility complex (MHC) antigen, was used in cryostat sections of aortic allografts.	bind
55948	3	8211	6	13	NULL	NULL	NULL	class II MHC antigen	GP		is homologous to					class II MHC antigen	GP	rabbit			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2515_s_81	9409222	43  As a marker of inflammation with activation of the immune system, the 2C4 monoclonal mouse-antirabbit antibody (Serotec, Oxford, England), which binds to the rabbit homologue of the class II major histocompatibility complex (MHC) antigen, was used in cryostat sections of aortic allografts.	bind
33126	1	8211	7	NULL	NULL	0	NULL	2C4 monoclonal mouse-antirabbit antibody 	NULL		binds to	NULL				class II MHC antigen	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2515_s_81	9409222	43  As a marker of inflammation with activation of the immune system, the 2C4 monoclonal mouse-antirabbit antibody (Serotec, Oxford, England), which binds to the rabbit homologue of the class II major histocompatibility complex (MHC) antigen, was used in cryostat sections of aortic allografts.	bind
33129	2	8211	7	NULL	NULL	0	NULL	class II MHC antigen	NULL		is homologous to	NULL				class II MHC antigen	NULL	rabbit			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2515_s_81	9409222	43  As a marker of inflammation with activation of the immune system, the 2C4 monoclonal mouse-antirabbit antibody (Serotec, Oxford, England), which binds to the rabbit homologue of the class II major histocompatibility complex (MHC) antigen, was used in cryostat sections of aortic allografts.	bind
33130	3	8211	7	NULL	NULL	0	NULL	MHC	NULL		is 	NULL				major histocompatibility complex	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2515_s_81	9409222	43  As a marker of inflammation with activation of the immune system, the 2C4 monoclonal mouse-antirabbit antibody (Serotec, Oxford, England), which binds to the rabbit homologue of the class II major histocompatibility complex (MHC) antigen, was used in cryostat sections of aortic allografts.	bind
27192	1	8212	6	13	NULL	NULL	NULL	S-1	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_5_471_s_148	9734469	43  In studies of the role of fsTnT in the regulation of myofilament activation, Schaertl et al 45  showed that TnT1 (residues 1 to 159) did not affect the rate of S-1 binding to actin in preparations reconstituted from myosin S-1 and regulated thin filaments.	bind
27193	2	8212	6	13	NULL	NULL	NULL	TnT1	GP		did not affect			1-159		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_5_471_s_148	9734469	43  In studies of the role of fsTnT in the regulation of myofilament activation, Schaertl et al 45  showed that TnT1 (residues 1 to 159) did not affect the rate of S-1 binding to actin in preparations reconstituted from myosin S-1 and regulated thin filaments.	bind
27194	3	8212	6	13	NULL	NULL	NULL	statement 2	Process		occurs in					myosin S-1	GP	 preparations reconstitued from			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_5_471_s_148	9734469	43  In studies of the role of fsTnT in the regulation of myofilament activation, Schaertl et al 45  showed that TnT1 (residues 1 to 159) did not affect the rate of S-1 binding to actin in preparations reconstituted from myosin S-1 and regulated thin filaments.	bind
27262	4	8212	6	13	NULL	NULL	NULL	statement 2	Process		occurs in					thin filaments	CellComponent	 preparations reconstitued from;;regulated			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_5_471_s_148	9734469	43  In studies of the role of fsTnT in the regulation of myofilament activation, Schaertl et al 45  showed that TnT1 (residues 1 to 159) did not affect the rate of S-1 binding to actin in preparations reconstituted from myosin S-1 and regulated thin filaments.	bind
33132	1	8212	7	NULL	NULL	0	NULL	S-1	NULL		bind	NULL				actin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_5_471_s_148	9734469	43  In studies of the role of fsTnT in the regulation of myofilament activation, Schaertl et al 45  showed that TnT1 (residues 1 to 159) did not affect the rate of S-1 binding to actin in preparations reconstituted from myosin S-1 and regulated thin filaments.	bind
33133	2	8212	7	NULL	NULL	0	NULL	S1	NULL		reconstituted from	NULL				myosin S-1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_5_471_s_148	9734469	43  In studies of the role of fsTnT in the regulation of myofilament activation, Schaertl et al 45  showed that TnT1 (residues 1 to 159) did not affect the rate of S-1 binding to actin in preparations reconstituted from myosin S-1 and regulated thin filaments.	bind
33134	3	8212	7	NULL	NULL	0	NULL	actin	NULL		reconstituted from	NULL				regulated thin filaments	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_5_471_s_148	9734469	43  In studies of the role of fsTnT in the regulation of myofilament activation, Schaertl et al 45  showed that TnT1 (residues 1 to 159) did not affect the rate of S-1 binding to actin in preparations reconstituted from myosin S-1 and regulated thin filaments.	bind
33135	4	8212	7	NULL	NULL	0	NULL	fsTnT 	NULL		regulates	NULL				myofilament	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_circulationres_83_5_471_s_148	9734469	43  In studies of the role of fsTnT in the regulation of myofilament activation, Schaertl et al 45  showed that TnT1 (residues 1 to 159) did not affect the rate of S-1 binding to actin in preparations reconstituted from myosin S-1 and regulated thin filaments.	bind
33136	5	8212	7	NULL	NULL	0	NULL	TnT1	NULL		does not affect	NULL		residues 1 to 159		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_5_471_s_148	9734469	43  In studies of the role of fsTnT in the regulation of myofilament activation, Schaertl et al 45  showed that TnT1 (residues 1 to 159) did not affect the rate of S-1 binding to actin in preparations reconstituted from myosin S-1 and regulated thin filaments.	bind
27263	1	8213	6	13	NULL	NULL	NULL	platelet	Cell		bind					neutrophils	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_2_372_s_155	9974421	43  Many studies have reported that other mechanisms may be implicated in platelet binding to neutrophils, such as (1) fibrinogen bridging via platelet GPIIb/IIa and neutrophil MAC-1, 44 45  (2) thrombospondin bridging via GPIa/Ia, GPIIb/IIa, or GPIV on platelets and a specific receptor on neutrophils, 46 47  (3) platelet ICAM-1 binding to neutrophil LFA-1, 48  and (4) immune complex interactions between platelet Fc RII (CD32) and neutrophil Fc RIIIb (CD16).	bind
27264	2	8213	6	13	NULL	NULL	NULL	platelet GPIIb/IIa	GP		bridges					fibrinogen	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_2_372_s_155	9974421	43  Many studies have reported that other mechanisms may be implicated in platelet binding to neutrophils, such as (1) fibrinogen bridging via platelet GPIIb/IIa and neutrophil MAC-1, 44 45  (2) thrombospondin bridging via GPIa/Ia, GPIIb/IIa, or GPIV on platelets and a specific receptor on neutrophils, 46 47  (3) platelet ICAM-1 binding to neutrophil LFA-1, 48  and (4) immune complex interactions between platelet Fc RII (CD32) and neutrophil Fc RIIIb (CD16).	bind
27265	3	8213	6	13	NULL	NULL	NULL	MAC-1	GP	neutrophil	bridges					fibrinogen	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_2_372_s_155	9974421	43  Many studies have reported that other mechanisms may be implicated in platelet binding to neutrophils, such as (1) fibrinogen bridging via platelet GPIIb/IIa and neutrophil MAC-1, 44 45  (2) thrombospondin bridging via GPIa/Ia, GPIIb/IIa, or GPIV on platelets and a specific receptor on neutrophils, 46 47  (3) platelet ICAM-1 binding to neutrophil LFA-1, 48  and (4) immune complex interactions between platelet Fc RII (CD32) and neutrophil Fc RIIIb (CD16).	bind
27535	4	8213	6	13	NULL	NULL	NULL	GPIa/Ia	GP		bridges					thrombospondin	GP				NULL	platelets	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_2_372_s_155	9974421	43  Many studies have reported that other mechanisms may be implicated in platelet binding to neutrophils, such as (1) fibrinogen bridging via platelet GPIIb/IIa and neutrophil MAC-1, 44 45  (2) thrombospondin bridging via GPIa/Ia, GPIIb/IIa, or GPIV on platelets and a specific receptor on neutrophils, 46 47  (3) platelet ICAM-1 binding to neutrophil LFA-1, 48  and (4) immune complex interactions between platelet Fc RII (CD32) and neutrophil Fc RIIIb (CD16).	bind
27536	5	8213	6	13	NULL	NULL	NULL	GPIIb/IIa	GP		bridges					thrombospondin	GP				NULL	platelets	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_2_372_s_155	9974421	43  Many studies have reported that other mechanisms may be implicated in platelet binding to neutrophils, such as (1) fibrinogen bridging via platelet GPIIb/IIa and neutrophil MAC-1, 44 45  (2) thrombospondin bridging via GPIa/Ia, GPIIb/IIa, or GPIV on platelets and a specific receptor on neutrophils, 46 47  (3) platelet ICAM-1 binding to neutrophil LFA-1, 48  and (4) immune complex interactions between platelet Fc RII (CD32) and neutrophil Fc RIIIb (CD16).	bind
27537	6	8213	6	13	NULL	NULL	NULL	GPIV	GP		bridges					thrombospondin	GP				NULL	platelets	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_2_372_s_155	9974421	43  Many studies have reported that other mechanisms may be implicated in platelet binding to neutrophils, such as (1) fibrinogen bridging via platelet GPIIb/IIa and neutrophil MAC-1, 44 45  (2) thrombospondin bridging via GPIa/Ia, GPIIb/IIa, or GPIV on platelets and a specific receptor on neutrophils, 46 47  (3) platelet ICAM-1 binding to neutrophil LFA-1, 48  and (4) immune complex interactions between platelet Fc RII (CD32) and neutrophil Fc RIIIb (CD16).	bind
27538	7	8213	6	13	NULL	NULL	NULL	ICAM-1	GP	platelet	bind					LFA-1	GP	neutrophil			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_2_372_s_155	9974421	43  Many studies have reported that other mechanisms may be implicated in platelet binding to neutrophils, such as (1) fibrinogen bridging via platelet GPIIb/IIa and neutrophil MAC-1, 44 45  (2) thrombospondin bridging via GPIa/Ia, GPIIb/IIa, or GPIV on platelets and a specific receptor on neutrophils, 46 47  (3) platelet ICAM-1 binding to neutrophil LFA-1, 48  and (4) immune complex interactions between platelet Fc RII (CD32) and neutrophil Fc RIIIb (CD16).	bind
27539	8	8213	6	13	NULL	NULL	NULL	Fc RII 	GP		is					CD32	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_2_372_s_155	9974421	43  Many studies have reported that other mechanisms may be implicated in platelet binding to neutrophils, such as (1) fibrinogen bridging via platelet GPIIb/IIa and neutrophil MAC-1, 44 45  (2) thrombospondin bridging via GPIa/Ia, GPIIb/IIa, or GPIV on platelets and a specific receptor on neutrophils, 46 47  (3) platelet ICAM-1 binding to neutrophil LFA-1, 48  and (4) immune complex interactions between platelet Fc RII (CD32) and neutrophil Fc RIIIb (CD16).	bind
27540	9	8213	6	13	NULL	NULL	NULL	Fc RIIIb	GP		is					CD16	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_2_372_s_155	9974421	43  Many studies have reported that other mechanisms may be implicated in platelet binding to neutrophils, such as (1) fibrinogen bridging via platelet GPIIb/IIa and neutrophil MAC-1, 44 45  (2) thrombospondin bridging via GPIa/Ia, GPIIb/IIa, or GPIV on platelets and a specific receptor on neutrophils, 46 47  (3) platelet ICAM-1 binding to neutrophil LFA-1, 48  and (4) immune complex interactions between platelet Fc RII (CD32) and neutrophil Fc RIIIb (CD16).	bind
27541	10	8213	6	13	NULL	NULL	NULL	Fc RII	GP	platelet	bind					Fc RIIIb	GP	neutrophil			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_2_372_s_155	9974421	43  Many studies have reported that other mechanisms may be implicated in platelet binding to neutrophils, such as (1) fibrinogen bridging via platelet GPIIb/IIa and neutrophil MAC-1, 44 45  (2) thrombospondin bridging via GPIa/Ia, GPIIb/IIa, or GPIV on platelets and a specific receptor on neutrophils, 46 47  (3) platelet ICAM-1 binding to neutrophil LFA-1, 48  and (4) immune complex interactions between platelet Fc RII (CD32) and neutrophil Fc RIIIb (CD16).	bind
55949	11	8213	6	13	NULL	NULL	NULL	GPIIb/IIa	GP	platelet	bridges					fibrinogen	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_2_372_s_155	9974421	43  Many studies have reported that other mechanisms may be implicated in platelet binding to neutrophils, such as (1) fibrinogen bridging via platelet GPIIb/IIa and neutrophil MAC-1, 44 45  (2) thrombospondin bridging via GPIa/Ia, GPIIb/IIa, or GPIV on platelets and a specific receptor on neutrophils, 46 47  (3) platelet ICAM-1 binding to neutrophil LFA-1, 48  and (4) immune complex interactions between platelet Fc RII (CD32) and neutrophil Fc RIIIb (CD16).	bind
33137	1	8213	7	NULL	NULL	0	NULL	platelet	NULL		bind	NULL				neutrophils	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_2_372_s_155	9974421	43  Many studies have reported that other mechanisms may be implicated in platelet binding to neutrophils, such as (1) fibrinogen bridging via platelet GPIIb/IIa and neutrophil MAC-1, 44 45  (2) thrombospondin bridging via GPIa/Ia, GPIIb/IIa, or GPIV on platelets and a specific receptor on neutrophils, 46 47  (3) platelet ICAM-1 binding to neutrophil LFA-1, 48  and (4) immune complex interactions between platelet Fc RII (CD32) and neutrophil Fc RIIIb (CD16).	bind
33138	2	8213	7	NULL	NULL	0	NULL	fibrinogen	NULL		bridging via	NULL				platelet GPIIb/IIa 	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_2_372_s_155	9974421	43  Many studies have reported that other mechanisms may be implicated in platelet binding to neutrophils, such as (1) fibrinogen bridging via platelet GPIIb/IIa and neutrophil MAC-1, 44 45  (2) thrombospondin bridging via GPIa/Ia, GPIIb/IIa, or GPIV on platelets and a specific receptor on neutrophils, 46 47  (3) platelet ICAM-1 binding to neutrophil LFA-1, 48  and (4) immune complex interactions between platelet Fc RII (CD32) and neutrophil Fc RIIIb (CD16).	bind
33139	3	8213	7	NULL	NULL	0	NULL	fibrinogen	NULL		bridging via	NULL				neutrophil MAC-1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_2_372_s_155	9974421	43  Many studies have reported that other mechanisms may be implicated in platelet binding to neutrophils, such as (1) fibrinogen bridging via platelet GPIIb/IIa and neutrophil MAC-1, 44 45  (2) thrombospondin bridging via GPIa/Ia, GPIIb/IIa, or GPIV on platelets and a specific receptor on neutrophils, 46 47  (3) platelet ICAM-1 binding to neutrophil LFA-1, 48  and (4) immune complex interactions between platelet Fc RII (CD32) and neutrophil Fc RIIIb (CD16).	bind
33140	4	8213	7	NULL	NULL	0	NULL	thrombospondin	NULL		bridging via	NULL				 GPIa/Ia	NULL				NULL	platelets	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_2_372_s_155	9974421	43  Many studies have reported that other mechanisms may be implicated in platelet binding to neutrophils, such as (1) fibrinogen bridging via platelet GPIIb/IIa and neutrophil MAC-1, 44 45  (2) thrombospondin bridging via GPIa/Ia, GPIIb/IIa, or GPIV on platelets and a specific receptor on neutrophils, 46 47  (3) platelet ICAM-1 binding to neutrophil LFA-1, 48  and (4) immune complex interactions between platelet Fc RII (CD32) and neutrophil Fc RIIIb (CD16).	bind
33141	5	8213	7	NULL	NULL	0	NULL	thrombospondin	NULL		bridging via	NULL				GPIIb/IIa	NULL				NULL	platelets	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_2_372_s_155	9974421	43  Many studies have reported that other mechanisms may be implicated in platelet binding to neutrophils, such as (1) fibrinogen bridging via platelet GPIIb/IIa and neutrophil MAC-1, 44 45  (2) thrombospondin bridging via GPIa/Ia, GPIIb/IIa, or GPIV on platelets and a specific receptor on neutrophils, 46 47  (3) platelet ICAM-1 binding to neutrophil LFA-1, 48  and (4) immune complex interactions between platelet Fc RII (CD32) and neutrophil Fc RIIIb (CD16).	bind
33142	6	8213	7	NULL	NULL	0	NULL	thrombospondin 	NULL		bridging via	NULL				 GPIV	NULL				NULL	platelets	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_2_372_s_155	9974421	43  Many studies have reported that other mechanisms may be implicated in platelet binding to neutrophils, such as (1) fibrinogen bridging via platelet GPIIb/IIa and neutrophil MAC-1, 44 45  (2) thrombospondin bridging via GPIa/Ia, GPIIb/IIa, or GPIV on platelets and a specific receptor on neutrophils, 46 47  (3) platelet ICAM-1 binding to neutrophil LFA-1, 48  and (4) immune complex interactions between platelet Fc RII (CD32) and neutrophil Fc RIIIb (CD16).	bind
33144	8	8213	7	10	NULL	0	NULL	platelet ICAM-1			bind					LFA-1		neutrophil			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_2_372_s_155	9974421	43  Many studies have reported that other mechanisms may be implicated in platelet binding to neutrophils, such as (1) fibrinogen bridging via platelet GPIIb/IIa and neutrophil MAC-1, 44 45  (2) thrombospondin bridging via GPIa/Ia, GPIIb/IIa, or GPIV on platelets and a specific receptor on neutrophils, 46 47  (3) platelet ICAM-1 binding to neutrophil LFA-1, 48  and (4) immune complex interactions between platelet Fc RII (CD32) and neutrophil Fc RIIIb (CD16).	bind
33145	9	8213	7	10	NULL	0	NULL	platelet Fc RII			interacts with					Fc RIIIb		neutrophil			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_2_372_s_155	9974421	43  Many studies have reported that other mechanisms may be implicated in platelet binding to neutrophils, such as (1) fibrinogen bridging via platelet GPIIb/IIa and neutrophil MAC-1, 44 45  (2) thrombospondin bridging via GPIa/Ia, GPIIb/IIa, or GPIV on platelets and a specific receptor on neutrophils, 46 47  (3) platelet ICAM-1 binding to neutrophil LFA-1, 48  and (4) immune complex interactions between platelet Fc RII (CD32) and neutrophil Fc RIIIb (CD16).	bind
33146	10	8213	7	NULL	NULL	0	NULL	statement 9	NULL		is a type of	NULL				immune complex interaction	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_2_372_s_155	9974421	43  Many studies have reported that other mechanisms may be implicated in platelet binding to neutrophils, such as (1) fibrinogen bridging via platelet GPIIb/IIa and neutrophil MAC-1, 44 45  (2) thrombospondin bridging via GPIa/Ia, GPIIb/IIa, or GPIV on platelets and a specific receptor on neutrophils, 46 47  (3) platelet ICAM-1 binding to neutrophil LFA-1, 48  and (4) immune complex interactions between platelet Fc RII (CD32) and neutrophil Fc RIIIb (CD16).	bind
33147	11	8213	7	10	NULL	0	NULL	Fc RII			is					CD32					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_2_372_s_155	9974421	43  Many studies have reported that other mechanisms may be implicated in platelet binding to neutrophils, such as (1) fibrinogen bridging via platelet GPIIb/IIa and neutrophil MAC-1, 44 45  (2) thrombospondin bridging via GPIa/Ia, GPIIb/IIa, or GPIV on platelets and a specific receptor on neutrophils, 46 47  (3) platelet ICAM-1 binding to neutrophil LFA-1, 48  and (4) immune complex interactions between platelet Fc RII (CD32) and neutrophil Fc RIIIb (CD16).	bind
33148	12	8213	7	10	NULL	0	NULL	Fc RIIIb			is					CD16					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_2_372_s_155	9974421	43  Many studies have reported that other mechanisms may be implicated in platelet binding to neutrophils, such as (1) fibrinogen bridging via platelet GPIIb/IIa and neutrophil MAC-1, 44 45  (2) thrombospondin bridging via GPIa/Ia, GPIIb/IIa, or GPIV on platelets and a specific receptor on neutrophils, 46 47  (3) platelet ICAM-1 binding to neutrophil LFA-1, 48  and (4) immune complex interactions between platelet Fc RII (CD32) and neutrophil Fc RIIIb (CD16).	bind
27542	1	8214	6	13	NULL	NULL	NULL	fibroblasts	Cell	human;; skin	unable to take					Ang II-LDL	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_97_s_202	8548433	43  The involvement of the scavenger receptor and not the LDL receptor in the uptake of Ang II - LDL by macrophages is supported by the following data: (1) Human skin fibroblasts (which lack the scavenger receptor) are unable to take up Ang II - LDL; (2) nonlabeled Ox-LDL, Ac-LDL, and fucoidin, which bind to the scavenger receptor but not native LDL, which binds to the LDL receptor, significantly compete with Ang II-125I - labeled LDL for its degradation by macrophages; and (3) Ang II - LDL, like Ac-LDL and Ox-LDL but unlike native LDL, does not bind to heparin.	bind
27543	2	8214	6	13	NULL	NULL	NULL	fibroblasts	Cell	human;; skin	lack					scavenger receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_97_s_202	8548433	43  The involvement of the scavenger receptor and not the LDL receptor in the uptake of Ang II - LDL by macrophages is supported by the following data: (1) Human skin fibroblasts (which lack the scavenger receptor) are unable to take up Ang II - LDL; (2) nonlabeled Ox-LDL, Ac-LDL, and fucoidin, which bind to the scavenger receptor but not native LDL, which binds to the LDL receptor, significantly compete with Ang II-125I - labeled LDL for its degradation by macrophages; and (3) Ang II - LDL, like Ac-LDL and Ox-LDL but unlike native LDL, does not bind to heparin.	bind
27544	3	8214	6	13	NULL	NULL	NULL	Ox-LDL	GP	nonlabeled	bind					scavenger receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_97_s_202	8548433	43  The involvement of the scavenger receptor and not the LDL receptor in the uptake of Ang II - LDL by macrophages is supported by the following data: (1) Human skin fibroblasts (which lack the scavenger receptor) are unable to take up Ang II - LDL; (2) nonlabeled Ox-LDL, Ac-LDL, and fucoidin, which bind to the scavenger receptor but not native LDL, which binds to the LDL receptor, significantly compete with Ang II-125I - labeled LDL for its degradation by macrophages; and (3) Ang II - LDL, like Ac-LDL and Ox-LDL but unlike native LDL, does not bind to heparin.	bind
27545	4	8214	6	13	NULL	NULL	NULL	Ac-LDL	GP	nonlabeled	bind					scavenger receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_97_s_202	8548433	43  The involvement of the scavenger receptor and not the LDL receptor in the uptake of Ang II - LDL by macrophages is supported by the following data: (1) Human skin fibroblasts (which lack the scavenger receptor) are unable to take up Ang II - LDL; (2) nonlabeled Ox-LDL, Ac-LDL, and fucoidin, which bind to the scavenger receptor but not native LDL, which binds to the LDL receptor, significantly compete with Ang II-125I - labeled LDL for its degradation by macrophages; and (3) Ang II - LDL, like Ac-LDL and Ox-LDL but unlike native LDL, does not bind to heparin.	bind
27546	5	8214	6	13	NULL	NULL	NULL	fucoidin	GP	nonlabeled	bind					scavenger receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_97_s_202	8548433	43  The involvement of the scavenger receptor and not the LDL receptor in the uptake of Ang II - LDL by macrophages is supported by the following data: (1) Human skin fibroblasts (which lack the scavenger receptor) are unable to take up Ang II - LDL; (2) nonlabeled Ox-LDL, Ac-LDL, and fucoidin, which bind to the scavenger receptor but not native LDL, which binds to the LDL receptor, significantly compete with Ang II-125I - labeled LDL for its degradation by macrophages; and (3) Ang II - LDL, like Ac-LDL and Ox-LDL but unlike native LDL, does not bind to heparin.	bind
27547	6	8214	6	13	NULL	NULL	NULL	LDL	GP	native	bind					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_97_s_202	8548433	43  The involvement of the scavenger receptor and not the LDL receptor in the uptake of Ang II - LDL by macrophages is supported by the following data: (1) Human skin fibroblasts (which lack the scavenger receptor) are unable to take up Ang II - LDL; (2) nonlabeled Ox-LDL, Ac-LDL, and fucoidin, which bind to the scavenger receptor but not native LDL, which binds to the LDL receptor, significantly compete with Ang II-125I - labeled LDL for its degradation by macrophages; and (3) Ang II - LDL, like Ac-LDL and Ox-LDL but unlike native LDL, does not bind to heparin.	bind
27548	7	8214	6	13	NULL	NULL	NULL	LDL	GP	Ang II-125I - labeled	is degraded by					macrophages	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_97_s_202	8548433	43  The involvement of the scavenger receptor and not the LDL receptor in the uptake of Ang II - LDL by macrophages is supported by the following data: (1) Human skin fibroblasts (which lack the scavenger receptor) are unable to take up Ang II - LDL; (2) nonlabeled Ox-LDL, Ac-LDL, and fucoidin, which bind to the scavenger receptor but not native LDL, which binds to the LDL receptor, significantly compete with Ang II-125I - labeled LDL for its degradation by macrophages; and (3) Ang II - LDL, like Ac-LDL and Ox-LDL but unlike native LDL, does not bind to heparin.	bind
27549	8	8214	6	13	NULL	NULL	NULL	Ang II - LDL	GP		does not bind					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_97_s_202	8548433	43  The involvement of the scavenger receptor and not the LDL receptor in the uptake of Ang II - LDL by macrophages is supported by the following data: (1) Human skin fibroblasts (which lack the scavenger receptor) are unable to take up Ang II - LDL; (2) nonlabeled Ox-LDL, Ac-LDL, and fucoidin, which bind to the scavenger receptor but not native LDL, which binds to the LDL receptor, significantly compete with Ang II-125I - labeled LDL for its degradation by macrophages; and (3) Ang II - LDL, like Ac-LDL and Ox-LDL but unlike native LDL, does not bind to heparin.	bind
27550	9	8214	6	13	NULL	NULL	NULL	Ac-LDL	GP		does not bind					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_97_s_202	8548433	43  The involvement of the scavenger receptor and not the LDL receptor in the uptake of Ang II - LDL by macrophages is supported by the following data: (1) Human skin fibroblasts (which lack the scavenger receptor) are unable to take up Ang II - LDL; (2) nonlabeled Ox-LDL, Ac-LDL, and fucoidin, which bind to the scavenger receptor but not native LDL, which binds to the LDL receptor, significantly compete with Ang II-125I - labeled LDL for its degradation by macrophages; and (3) Ang II - LDL, like Ac-LDL and Ox-LDL but unlike native LDL, does not bind to heparin.	bind
27551	10	8214	6	13	NULL	NULL	NULL	Ox-LDL	GP		does not bind					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_97_s_202	8548433	43  The involvement of the scavenger receptor and not the LDL receptor in the uptake of Ang II - LDL by macrophages is supported by the following data: (1) Human skin fibroblasts (which lack the scavenger receptor) are unable to take up Ang II - LDL; (2) nonlabeled Ox-LDL, Ac-LDL, and fucoidin, which bind to the scavenger receptor but not native LDL, which binds to the LDL receptor, significantly compete with Ang II-125I - labeled LDL for its degradation by macrophages; and (3) Ang II - LDL, like Ac-LDL and Ox-LDL but unlike native LDL, does not bind to heparin.	bind
27552	11	8214	6	13	NULL	NULL	NULL	LDL	GP	native	bind					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_97_s_202	8548433	43  The involvement of the scavenger receptor and not the LDL receptor in the uptake of Ang II - LDL by macrophages is supported by the following data: (1) Human skin fibroblasts (which lack the scavenger receptor) are unable to take up Ang II - LDL; (2) nonlabeled Ox-LDL, Ac-LDL, and fucoidin, which bind to the scavenger receptor but not native LDL, which binds to the LDL receptor, significantly compete with Ang II-125I - labeled LDL for its degradation by macrophages; and (3) Ang II - LDL, like Ac-LDL and Ox-LDL but unlike native LDL, does not bind to heparin.	bind
33149	1	8214	7	NULL	NULL	0	NULL	Ang II - LDL	NULL		uptake by	NULL				macrophages	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_97_s_202	8548433	43  The involvement of the scavenger receptor and not the LDL receptor in the uptake of Ang II - LDL by macrophages is supported by the following data: (1) Human skin fibroblasts (which lack the scavenger receptor) are unable to take up Ang II - LDL; (2) nonlabeled Ox-LDL, Ac-LDL, and fucoidin, which bind to the scavenger receptor but not native LDL, which binds to the LDL receptor, significantly compete with Ang II-125I - labeled LDL for its degradation by macrophages; and (3) Ang II - LDL, like Ac-LDL and Ox-LDL but unlike native LDL, does not bind to heparin.	bind
33150	2	8214	7	NULL	NULL	0	NULL	LDL receptor	NULL		is not involved in	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_97_s_202	8548433	43  The involvement of the scavenger receptor and not the LDL receptor in the uptake of Ang II - LDL by macrophages is supported by the following data: (1) Human skin fibroblasts (which lack the scavenger receptor) are unable to take up Ang II - LDL; (2) nonlabeled Ox-LDL, Ac-LDL, and fucoidin, which bind to the scavenger receptor but not native LDL, which binds to the LDL receptor, significantly compete with Ang II-125I - labeled LDL for its degradation by macrophages; and (3) Ang II - LDL, like Ac-LDL and Ox-LDL but unlike native LDL, does not bind to heparin.	bind
33152	3	8214	7	NULL	NULL	0	NULL	scavenger receptor	NULL		is involved in	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_97_s_202	8548433	43  The involvement of the scavenger receptor and not the LDL receptor in the uptake of Ang II - LDL by macrophages is supported by the following data: (1) Human skin fibroblasts (which lack the scavenger receptor) are unable to take up Ang II - LDL; (2) nonlabeled Ox-LDL, Ac-LDL, and fucoidin, which bind to the scavenger receptor but not native LDL, which binds to the LDL receptor, significantly compete with Ang II-125I - labeled LDL for its degradation by macrophages; and (3) Ang II - LDL, like Ac-LDL and Ox-LDL but unlike native LDL, does not bind to heparin.	bind
33153	4	8214	7	10	NULL	0	NULL	fibroblasts 		human;;skin	lacks					scavenger receptor					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_97_s_202	8548433	43  The involvement of the scavenger receptor and not the LDL receptor in the uptake of Ang II - LDL by macrophages is supported by the following data: (1) Human skin fibroblasts (which lack the scavenger receptor) are unable to take up Ang II - LDL; (2) nonlabeled Ox-LDL, Ac-LDL, and fucoidin, which bind to the scavenger receptor but not native LDL, which binds to the LDL receptor, significantly compete with Ang II-125I - labeled LDL for its degradation by macrophages; and (3) Ang II - LDL, like Ac-LDL and Ox-LDL but unlike native LDL, does not bind to heparin.	bind
33154	5	8214	7	10	NULL	0	NULL	fibroblasts 		human;;skin	unable to takeup					AngII - LDL					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_97_s_202	8548433	43  The involvement of the scavenger receptor and not the LDL receptor in the uptake of Ang II - LDL by macrophages is supported by the following data: (1) Human skin fibroblasts (which lack the scavenger receptor) are unable to take up Ang II - LDL; (2) nonlabeled Ox-LDL, Ac-LDL, and fucoidin, which bind to the scavenger receptor but not native LDL, which binds to the LDL receptor, significantly compete with Ang II-125I - labeled LDL for its degradation by macrophages; and (3) Ang II - LDL, like Ac-LDL and Ox-LDL but unlike native LDL, does not bind to heparin.	bind
33155	6	8214	7	NULL	NULL	0	NULL	Ox-LDL	NULL	nonlabeled	binds to	NULL				scavenger receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_97_s_202	8548433	43  The involvement of the scavenger receptor and not the LDL receptor in the uptake of Ang II - LDL by macrophages is supported by the following data: (1) Human skin fibroblasts (which lack the scavenger receptor) are unable to take up Ang II - LDL; (2) nonlabeled Ox-LDL, Ac-LDL, and fucoidin, which bind to the scavenger receptor but not native LDL, which binds to the LDL receptor, significantly compete with Ang II-125I - labeled LDL for its degradation by macrophages; and (3) Ang II - LDL, like Ac-LDL and Ox-LDL but unlike native LDL, does not bind to heparin.	bind
33156	7	8214	7	NULL	NULL	0	NULL	Ac-LDL	NULL		binds to	NULL				scavenger receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_97_s_202	8548433	43  The involvement of the scavenger receptor and not the LDL receptor in the uptake of Ang II - LDL by macrophages is supported by the following data: (1) Human skin fibroblasts (which lack the scavenger receptor) are unable to take up Ang II - LDL; (2) nonlabeled Ox-LDL, Ac-LDL, and fucoidin, which bind to the scavenger receptor but not native LDL, which binds to the LDL receptor, significantly compete with Ang II-125I - labeled LDL for its degradation by macrophages; and (3) Ang II - LDL, like Ac-LDL and Ox-LDL but unlike native LDL, does not bind to heparin.	bind
33157	8	8214	7	NULL	NULL	0	NULL	fucoidin	NULL		binds to	NULL				scavenger receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_97_s_202	8548433	43  The involvement of the scavenger receptor and not the LDL receptor in the uptake of Ang II - LDL by macrophages is supported by the following data: (1) Human skin fibroblasts (which lack the scavenger receptor) are unable to take up Ang II - LDL; (2) nonlabeled Ox-LDL, Ac-LDL, and fucoidin, which bind to the scavenger receptor but not native LDL, which binds to the LDL receptor, significantly compete with Ang II-125I - labeled LDL for its degradation by macrophages; and (3) Ang II - LDL, like Ac-LDL and Ox-LDL but unlike native LDL, does not bind to heparin.	bind
33158	9	8214	7	NULL	NULL	0	NULL	LDL	NULL	native	does not bind	NULL				scavenger receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_97_s_202	8548433	43  The involvement of the scavenger receptor and not the LDL receptor in the uptake of Ang II - LDL by macrophages is supported by the following data: (1) Human skin fibroblasts (which lack the scavenger receptor) are unable to take up Ang II - LDL; (2) nonlabeled Ox-LDL, Ac-LDL, and fucoidin, which bind to the scavenger receptor but not native LDL, which binds to the LDL receptor, significantly compete with Ang II-125I - labeled LDL for its degradation by macrophages; and (3) Ang II - LDL, like Ac-LDL and Ox-LDL but unlike native LDL, does not bind to heparin.	bind
33159	10	8214	7	NULL	NULL	0	NULL	LDL	NULL		binds to	NULL				LDL receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_97_s_202	8548433	43  The involvement of the scavenger receptor and not the LDL receptor in the uptake of Ang II - LDL by macrophages is supported by the following data: (1) Human skin fibroblasts (which lack the scavenger receptor) are unable to take up Ang II - LDL; (2) nonlabeled Ox-LDL, Ac-LDL, and fucoidin, which bind to the scavenger receptor but not native LDL, which binds to the LDL receptor, significantly compete with Ang II-125I - labeled LDL for its degradation by macrophages; and (3) Ang II - LDL, like Ac-LDL and Ox-LDL but unlike native LDL, does not bind to heparin.	bind
33160	11	8214	7	NULL	NULL	0	NULL	macrophages	NULL		degrade	NULL				Ang II-125I - labeled LDL	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_97_s_202	8548433	43  The involvement of the scavenger receptor and not the LDL receptor in the uptake of Ang II - LDL by macrophages is supported by the following data: (1) Human skin fibroblasts (which lack the scavenger receptor) are unable to take up Ang II - LDL; (2) nonlabeled Ox-LDL, Ac-LDL, and fucoidin, which bind to the scavenger receptor but not native LDL, which binds to the LDL receptor, significantly compete with Ang II-125I - labeled LDL for its degradation by macrophages; and (3) Ang II - LDL, like Ac-LDL and Ox-LDL but unlike native LDL, does not bind to heparin.	bind
33161	13	8214	7	NULL	NULL	0	NULL	statement 11	NULL		compete with	NULL				statement 12	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_97_s_202	8548433	43  The involvement of the scavenger receptor and not the LDL receptor in the uptake of Ang II - LDL by macrophages is supported by the following data: (1) Human skin fibroblasts (which lack the scavenger receptor) are unable to take up Ang II - LDL; (2) nonlabeled Ox-LDL, Ac-LDL, and fucoidin, which bind to the scavenger receptor but not native LDL, which binds to the LDL receptor, significantly compete with Ang II-125I - labeled LDL for its degradation by macrophages; and (3) Ang II - LDL, like Ac-LDL and Ox-LDL but unlike native LDL, does not bind to heparin.	bind
33163	14	8214	7	NULL	NULL	0	NULL	Ang II - LDL	NULL		does not bind	NULL				heparin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_97_s_202	8548433	43  The involvement of the scavenger receptor and not the LDL receptor in the uptake of Ang II - LDL by macrophages is supported by the following data: (1) Human skin fibroblasts (which lack the scavenger receptor) are unable to take up Ang II - LDL; (2) nonlabeled Ox-LDL, Ac-LDL, and fucoidin, which bind to the scavenger receptor but not native LDL, which binds to the LDL receptor, significantly compete with Ang II-125I - labeled LDL for its degradation by macrophages; and (3) Ang II - LDL, like Ac-LDL and Ox-LDL but unlike native LDL, does not bind to heparin.	bind
33164	15	8214	7	NULL	NULL	0	NULL	Ac-LDL	NULL		does not bind	NULL				heparin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_97_s_202	8548433	43  The involvement of the scavenger receptor and not the LDL receptor in the uptake of Ang II - LDL by macrophages is supported by the following data: (1) Human skin fibroblasts (which lack the scavenger receptor) are unable to take up Ang II - LDL; (2) nonlabeled Ox-LDL, Ac-LDL, and fucoidin, which bind to the scavenger receptor but not native LDL, which binds to the LDL receptor, significantly compete with Ang II-125I - labeled LDL for its degradation by macrophages; and (3) Ang II - LDL, like Ac-LDL and Ox-LDL but unlike native LDL, does not bind to heparin.	bind
33165	16	8214	7	NULL	NULL	0	NULL	Ox-LDL	NULL		does not bind	NULL				heparin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_97_s_202	8548433	43  The involvement of the scavenger receptor and not the LDL receptor in the uptake of Ang II - LDL by macrophages is supported by the following data: (1) Human skin fibroblasts (which lack the scavenger receptor) are unable to take up Ang II - LDL; (2) nonlabeled Ox-LDL, Ac-LDL, and fucoidin, which bind to the scavenger receptor but not native LDL, which binds to the LDL receptor, significantly compete with Ang II-125I - labeled LDL for its degradation by macrophages; and (3) Ang II - LDL, like Ac-LDL and Ox-LDL but unlike native LDL, does not bind to heparin.	bind
33168	17	8214	7	NULL	NULL	0	NULL	LDL	NULL	native	bind	NULL				heparin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_97_s_202	8548433	43  The involvement of the scavenger receptor and not the LDL receptor in the uptake of Ang II - LDL by macrophages is supported by the following data: (1) Human skin fibroblasts (which lack the scavenger receptor) are unable to take up Ang II - LDL; (2) nonlabeled Ox-LDL, Ac-LDL, and fucoidin, which bind to the scavenger receptor but not native LDL, which binds to the LDL receptor, significantly compete with Ang II-125I - labeled LDL for its degradation by macrophages; and (3) Ang II - LDL, like Ac-LDL and Ox-LDL but unlike native LDL, does not bind to heparin.	bind
33170	12	8214	7	NULL	NULL	0	NULL	macrophages	NULL		degrade	NULL				LDL	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_1_97_s_202	8548433	43  The involvement of the scavenger receptor and not the LDL receptor in the uptake of Ang II - LDL by macrophages is supported by the following data: (1) Human skin fibroblasts (which lack the scavenger receptor) are unable to take up Ang II - LDL; (2) nonlabeled Ox-LDL, Ac-LDL, and fucoidin, which bind to the scavenger receptor but not native LDL, which binds to the LDL receptor, significantly compete with Ang II-125I - labeled LDL for its degradation by macrophages; and (3) Ang II - LDL, like Ac-LDL and Ox-LDL but unlike native LDL, does not bind to heparin.	bind
27266	1	8215	6	13	NULL	NULL	NULL	TM	GP		interacts with					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_1_47_s_276	10400910	43  Thus, the increase in the Ca2+ sensitivity of the FHC myofilaments could be due to the changes in the cooperative activation of thin filaments by altering the interaction of TM and actin, by affecting the TnT binding to TM, or through both mechanisms.	bind
27267	2	8215	6	13	NULL	NULL	NULL	TnT	GP		bind					TM	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_1_47_s_276	10400910	43  Thus, the increase in the Ca2+ sensitivity of the FHC myofilaments could be due to the changes in the cooperative activation of thin filaments by altering the interaction of TM and actin, by affecting the TnT binding to TM, or through both mechanisms.	bind
27268	3	8215	6	13	NULL	NULL	NULL	Ca+2 sensitivity	Process		increased in					FHC myofilaments	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_1_47_s_276	10400910	43  Thus, the increase in the Ca2+ sensitivity of the FHC myofilaments could be due to the changes in the cooperative activation of thin filaments by altering the interaction of TM and actin, by affecting the TnT binding to TM, or through both mechanisms.	bind
27269	4	8215	6	13	NULL	NULL	NULL	statement 3	Process		occur due to		may			statement 1	Process	alteration of 			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_1_47_s_276	10400910	43  Thus, the increase in the Ca2+ sensitivity of the FHC myofilaments could be due to the changes in the cooperative activation of thin filaments by altering the interaction of TM and actin, by affecting the TnT binding to TM, or through both mechanisms.	bind
27553	5	8215	6	13	NULL	NULL	NULL	statement 3	Process		occur due to		may			statement 2	Process	alteration of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_1_47_s_276	10400910	43  Thus, the increase in the Ca2+ sensitivity of the FHC myofilaments could be due to the changes in the cooperative activation of thin filaments by altering the interaction of TM and actin, by affecting the TnT binding to TM, or through both mechanisms.	bind
27554	6	8215	6	13	NULL	NULL	NULL	statement 4	Process		acts in cooperation with		may			statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_1_47_s_276	10400910	43  Thus, the increase in the Ca2+ sensitivity of the FHC myofilaments could be due to the changes in the cooperative activation of thin filaments by altering the interaction of TM and actin, by affecting the TnT binding to TM, or through both mechanisms.	bind
33176	1	8215	7	NULL	NULL	0	NULL	TM	NULL		interacts with	NULL				actin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_85_1_47_s_276	10400910	43  Thus, the increase in the Ca2+ sensitivity of the FHC myofilaments could be due to the changes in the cooperative activation of thin filaments by altering the interaction of TM and actin, by affecting the TnT binding to TM, or through both mechanisms.	bind
33177	2	8215	7	NULL	NULL	0	NULL	TnT	NULL		bind	NULL				TM	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_85_1_47_s_276	10400910	43  Thus, the increase in the Ca2+ sensitivity of the FHC myofilaments could be due to the changes in the cooperative activation of thin filaments by altering the interaction of TM and actin, by affecting the TnT binding to TM, or through both mechanisms.	bind
33178	3	8215	7	NULL	NULL	0	NULL	Ca2+ sensitivity	NULL		increase in	NULL				FHC myofilaments	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_85_1_47_s_276	10400910	43  Thus, the increase in the Ca2+ sensitivity of the FHC myofilaments could be due to the changes in the cooperative activation of thin filaments by altering the interaction of TM and actin, by affecting the TnT binding to TM, or through both mechanisms.	bind
33180	4	8215	7	NULL	NULL	0	NULL	statement 3	NULL		due to changes in	NULL				thin filaments	NULL	cooperative activation of			NULL		0	NULL	NULL	NULL	gw60_circulationres_85_1_47_s_276	10400910	43  Thus, the increase in the Ca2+ sensitivity of the FHC myofilaments could be due to the changes in the cooperative activation of thin filaments by altering the interaction of TM and actin, by affecting the TnT binding to TM, or through both mechanisms.	bind
33182	5	8215	7	NULL	NULL	0	NULL	statement 4	NULL		occur by altering	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_85_1_47_s_276	10400910	43  Thus, the increase in the Ca2+ sensitivity of the FHC myofilaments could be due to the changes in the cooperative activation of thin filaments by altering the interaction of TM and actin, by affecting the TnT binding to TM, or through both mechanisms.	bind
33183	6	8215	7	NULL	NULL	0	NULL	statement 4	NULL		occur by affecting	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_1_47_s_276	10400910	43  Thus, the increase in the Ca2+ sensitivity of the FHC myofilaments could be due to the changes in the cooperative activation of thin filaments by altering the interaction of TM and actin, by affecting the TnT binding to TM, or through both mechanisms.	bind
33185	7	8215	7	NULL	NULL	0	NULL	statement 5	NULL		in simultaneous with	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_85_1_47_s_276	10400910	43  Thus, the increase in the Ca2+ sensitivity of the FHC myofilaments could be due to the changes in the cooperative activation of thin filaments by altering the interaction of TM and actin, by affecting the TnT binding to TM, or through both mechanisms.	bind
33186	8	8215	7	NULL	NULL	0	NULL	statement 5	NULL		is an alternative to	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_85_1_47_s_276	10400910	43  Thus, the increase in the Ca2+ sensitivity of the FHC myofilaments could be due to the changes in the cooperative activation of thin filaments by altering the interaction of TM and actin, by affecting the TnT binding to TM, or through both mechanisms.	bind
33187	9	8215	7	NULL	NULL	0	NULL	statement 6	NULL		is an alternative to	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_85_1_47_s_276	10400910	43  Thus, the increase in the Ca2+ sensitivity of the FHC myofilaments could be due to the changes in the cooperative activation of thin filaments by altering the interaction of TM and actin, by affecting the TnT binding to TM, or through both mechanisms.	bind
27270	1	8216	6	13	NULL	NULL	NULL	HSP90	GP		bind					ADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_25_3473_s_213	15967841	43 Moreover, HSP90 function is sensitive to the cellular energy charge, as HSP90 readily binds ADP, and this event promotes client protein degradation.	bind
27271	2	8216	6	13	NULL	NULL	NULL	statement 1	Process		promotes					HSP90	GP	degradation of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_25_3473_s_213	15967841	43 Moreover, HSP90 function is sensitive to the cellular energy charge, as HSP90 readily binds ADP, and this event promotes client protein degradation.	bind
27272	3	8216	6	13	NULL	NULL	NULL	HSP90	GP	function of	is sensitive to					energy charge		cellular			NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_25_3473_s_213	15967841	43 Moreover, HSP90 function is sensitive to the cellular energy charge, as HSP90 readily binds ADP, and this event promotes client protein degradation.	bind
33192	1	8216	7	10	NULL	0	NULL	HSP90		function of	is sensitive to					cellular energy charge					NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_25_3473_s_213	15967841	43 Moreover, HSP90 function is sensitive to the cellular energy charge, as HSP90 readily binds ADP, and this event promotes client protein degradation.	bind
33193	2	8216	7	NULL	NULL	0	NULL	HSP90	NULL		binds	NULL				ADP	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_111_25_3473_s_213	15967841	43 Moreover, HSP90 function is sensitive to the cellular energy charge, as HSP90 readily binds ADP, and this event promotes client protein degradation.	bind
33194	3	8216	7	NULL	NULL	0	NULL	statement 2	NULL		promotes	NULL				client protein	NULL	degradation of			NULL		0	NULL	NULL	NULL	gw70_circulation_111_25_3473_s_213	15967841	43 Moreover, HSP90 function is sensitive to the cellular energy charge, as HSP90 readily binds ADP, and this event promotes client protein degradation.	bind
27273	1	8217	6	13	NULL	NULL	NULL	angiotensin II	GP		induces					SMC marker gene	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_131	15718508	43,44  In addition, angiotensin II - induced activation of SMC marker gene expression has  also been shown to be dependent on Prx1, a homeodomain protein shown to dramatically  increase SRF binding to the highly conserved degenerate CArG elements found in the  promoter region of most SMC marker genes.	bind
27274	2	8217	6	13	NULL	NULL	NULL	statement 1	Process		is dependent on					Prx1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_131	15718508	43,44  In addition, angiotensin II - induced activation of SMC marker gene expression has  also been shown to be dependent on Prx1, a homeodomain protein shown to dramatically  increase SRF binding to the highly conserved degenerate CArG elements found in the  promoter region of most SMC marker genes.	bind
27275	3	8217	6	13	NULL	NULL	NULL	Prx1	GP		is a type of					homeodomain protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_131	15718508	43,44  In addition, angiotensin II - induced activation of SMC marker gene expression has  also been shown to be dependent on Prx1, a homeodomain protein shown to dramatically  increase SRF binding to the highly conserved degenerate CArG elements found in the  promoter region of most SMC marker genes.	bind
27276	4	8217	6	13	NULL	NULL	NULL	SRF	GP		bind					SMC marker gene	GP			CArG element of promoter	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_131	15718508	43,44  In addition, angiotensin II - induced activation of SMC marker gene expression has  also been shown to be dependent on Prx1, a homeodomain protein shown to dramatically  increase SRF binding to the highly conserved degenerate CArG elements found in the  promoter region of most SMC marker genes.	bind
27277	5	8217	6	13	NULL	NULL	NULL	Prx1	GP		increases					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_131	15718508	43,44  In addition, angiotensin II - induced activation of SMC marker gene expression has  also been shown to be dependent on Prx1, a homeodomain protein shown to dramatically  increase SRF binding to the highly conserved degenerate CArG elements found in the  promoter region of most SMC marker genes.	bind
33195	1	8217	7	NULL	NULL	0	NULL	angiotensin II	NULL		induce	NULL				SMC marker gene	NULL	activation of			NULL		0	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_131	15718508	43,44  In addition, angiotensin II - induced activation of SMC marker gene expression has  also been shown to be dependent on Prx1, a homeodomain protein shown to dramatically  increase SRF binding to the highly conserved degenerate CArG elements found in the  promoter region of most SMC marker genes.	bind
33196	2	8217	7	NULL	NULL	0	NULL	statement 1	NULL		depends on	NULL				Prx1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_131	15718508	43,44  In addition, angiotensin II - induced activation of SMC marker gene expression has  also been shown to be dependent on Prx1, a homeodomain protein shown to dramatically  increase SRF binding to the highly conserved degenerate CArG elements found in the  promoter region of most SMC marker genes.	bind
33197	3	8217	7	NULL	NULL	0	NULL	Prx1	NULL		is a type of	NULL				homeodomain protein	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_131	15718508	43,44  In addition, angiotensin II - induced activation of SMC marker gene expression has  also been shown to be dependent on Prx1, a homeodomain protein shown to dramatically  increase SRF binding to the highly conserved degenerate CArG elements found in the  promoter region of most SMC marker genes.	bind
33198	4	8217	7	NULL	NULL	0	NULL	SRF	NULL		bind	NULL				SMC marker gene	NULL			highly conserved degenerate CArG elements	NULL		0	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_131	15718508	43,44  In addition, angiotensin II - induced activation of SMC marker gene expression has  also been shown to be dependent on Prx1, a homeodomain protein shown to dramatically  increase SRF binding to the highly conserved degenerate CArG elements found in the  promoter region of most SMC marker genes.	bind
33199	5	8217	7	NULL	NULL	0	NULL	Prx1	NULL		increase	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_131	15718508	43,44  In addition, angiotensin II - induced activation of SMC marker gene expression has  also been shown to be dependent on Prx1, a homeodomain protein shown to dramatically  increase SRF binding to the highly conserved degenerate CArG elements found in the  promoter region of most SMC marker genes.	bind
27278	1	8218	6	13	NULL	NULL	NULL	VASP	GP		bind					c-Abl	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1403_s_149	15178555	43,44  VASP binding to c-Abl might be involved in regulation of c-Abl activity, which may then regulate cell growth.	bind
27279	2	8218	6	13	NULL	NULL	NULL	statement 1	Process		is involved in		may			c-Abl activity	GP	regulation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1403_s_149	15178555	43,44  VASP binding to c-Abl might be involved in regulation of c-Abl activity, which may then regulate cell growth.	bind
27280	3	8218	6	13	NULL	NULL	NULL	statement 2	Process		regulate		may			cell growth	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1403_s_149	15178555	43,44  VASP binding to c-Abl might be involved in regulation of c-Abl activity, which may then regulate cell growth.	bind
33201	1	8218	7	NULL	NULL	0	NULL	VASP	NULL		bind	NULL				 c-Abl	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1403_s_149	15178555	43,44  VASP binding to c-Abl might be involved in regulation of c-Abl activity, which may then regulate cell growth.	bind
33203	2	8218	7	10	NULL	0	NULL	statement 1			is involved in		might			c-Abl activity		regulation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1403_s_149	15178555	43,44  VASP binding to c-Abl might be involved in regulation of c-Abl activity, which may then regulate cell growth.	bind
33205	3	8218	7	10	NULL	0	NULL	statement 2			regulate 		may			cell growth					NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_8_1403_s_149	15178555	43,44  VASP binding to c-Abl might be involved in regulation of c-Abl activity, which may then regulate cell growth.	bind
27281	1	8219	6	13	NULL	NULL	NULL	GST-HPV16 L2	GP		bind			1-128		GSTrap FF	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_14_12546_s_42	12560332	43-kDa Protein Purification and Identification-- GST-HPV16 L2-(1-128)-GFP was bound to a GSTrap FF column, and detergent extracts  of 109 SiHa cells in buffer A were passed over the column.	bind
33209	1	8219	7	10	NULL	0	NULL	GST-HPV16 L2			bind			1-128		GSTrap FF					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_14_12546_s_42	12560332	43-kDa Protein Purification and Identification-- GST-HPV16 L2-(1-128)-GFP was bound to a GSTrap FF column, and detergent extracts  of 109 SiHa cells in buffer A were passed over the column.	bind
27282	1	8221	6	13	NULL	NULL	NULL	Synaptotagmin	GP		bind			C2B domain		AP-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_nature_434_7031_409_s_238	15772668	436, 4 16 (2001) |  Article |  PubMed |  ISI |  ChemPort |                         Chapman, E. R., Desai, R. C., Davis, A. F. & Tornehl, C. K. Delineation of the  oligomerization, AP-2 binding, and synprint binding region of the C2B domain of synaptotagmin.	bind
33214	1	8221	7	10	NULL	0	NULL	synaptotagmin			bind			C2B domain		AP-2					NULL		NULL	NULL	NULL	NULL	gw70_nature_434_7031_409_s_238	15772668	436, 4 16 (2001) |  Article |  PubMed |  ISI |  ChemPort |                         Chapman, E. R., Desai, R. C., Davis, A. F. & Tornehl, C. K. Delineation of the  oligomerization, AP-2 binding, and synprint binding region of the C2B domain of synaptotagmin.	bind
27284	1	8222	6	13	NULL	NULL	NULL	retinoblastoma protein	GP		bind					E2F residues	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3439_s_438	11504882	44       Hagemeier,C., Cook,A. and Kouzarides,T. (1993) The retinoblastoma protein binds E2F residues required for activation  in vivo and TBP binding  in vitro.	bind
27285	2	8222	6	13	NULL	NULL	NULL	statement 1	Process		is required for					activation	Process				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3439_s_438	11504882	44       Hagemeier,C., Cook,A. and Kouzarides,T. (1993) The retinoblastoma protein binds E2F residues required for activation  in vivo and TBP binding  in vitro.	bind
27286	3	8222	6	13	NULL	NULL	NULL	statement 1	Process		bind					TBP	GP	binding of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3439_s_438	11504882	44       Hagemeier,C., Cook,A. and Kouzarides,T. (1993) The retinoblastoma protein binds E2F residues required for activation  in vivo and TBP binding  in vitro.	bind
33215	1	8222	7	NULL	NULL	0	NULL	 retinoblastoma protein	NULL		bind	NULL				E2F residues	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3439_s_438	11504882	44       Hagemeier,C., Cook,A. and Kouzarides,T. (1993) The retinoblastoma protein binds E2F residues required for activation  in vivo and TBP binding  in vitro.	bind
33216	2	8222	7	NULL	NULL	0	NULL	statement 1	NULL		is required for	NULL				activation	NULL				NULL	in vivo	0	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3439_s_438	11504882	44       Hagemeier,C., Cook,A. and Kouzarides,T. (1993) The retinoblastoma protein binds E2F residues required for activation  in vivo and TBP binding  in vitro.	bind
33217	3	8222	7	NULL	NULL	0	NULL	statement 1	NULL		is required for	NULL				TBP	NULL	binding of			NULL	in vitro	0	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3439_s_438	11504882	44       Hagemeier,C., Cook,A. and Kouzarides,T. (1993) The retinoblastoma protein binds E2F residues required for activation  in vivo and TBP binding  in vitro.	bind
27287	1	8223	6	13	NULL	NULL	NULL	ribosomal protein S8	GP	Escherichia coli	bind					16S rRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_447_s_458	11788706	44       Mougel,M., Ehresmann,B. and Ehresmann C. (1986) Binding of  Escherichia coli ribosomal protein S8 to 16S rRNA: kinetic and thermodynamic characterization.	bind
33218	1	8223	7	NULL	NULL	0	NULL	ribosomal protein S8 	NULL	Escherichia coli	bind	NULL				16S rRNA	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_447_s_458	11788706	44       Mougel,M., Ehresmann,B. and Ehresmann C. (1986) Binding of  Escherichia coli ribosomal protein S8 to 16S rRNA: kinetic and thermodynamic characterization.	bind
27288	1	8224	6	13	NULL	NULL	NULL	RBP-Jkappa/CBF1	GP	thymic	bind									NF-kappaB-like element	NULL	thymus nuclear extracts	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_11_2284_s_357	11376147	44       Shirakata,Y., Shuman,J.D. and Coligan,J.E. (1996) Purification of a novel MHC class I element binding activity from thymus nuclear extracts reveals that thymic RBP-Jkappa/CBF1 binds to NF-kappaB-like elements.	bind
33219	1	8224	7	NULL	NULL	0	NULL	 RBP-Jkappa/CBF1	NULL	thymic	binds	NULL					NULL			NF-kappaB-like elements	NULL	thymus nuclear extracts 	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_11_2284_s_357	11376147	44       Shirakata,Y., Shuman,J.D. and Coligan,J.E. (1996) Purification of a novel MHC class I element binding activity from thymus nuclear extracts reveals that thymic RBP-Jkappa/CBF1 binds to NF-kappaB-like elements.	bind
27289	1	8225	6	13	NULL	NULL	NULL	CRP	GP	Aggregated	bind		selectively			LDL	GP				NULL	whole plasma	NULL	NULL	NULL	NULL	gw60_circulation_99_2_237_s_139	9892589	44  45  Aggregated but not soluble native CRP selectively binds LDL and VLDL from whole plasma and, as we have previously proposed, could thereby participate in their atherogenic accumulation.	bind
27290	2	8225	6	13	NULL	NULL	NULL	CRP	GP	Aggregated	bind		selectively			VLDL	GP				NULL	whole plasma	NULL	NULL	NULL	NULL	gw60_circulation_99_2_237_s_139	9892589	44  45  Aggregated but not soluble native CRP selectively binds LDL and VLDL from whole plasma and, as we have previously proposed, could thereby participate in their atherogenic accumulation.	bind
55950	3	8225	6	13	NULL	NULL	NULL	CRP	GP	soluble;;native	does not bind					LDL	GP				NULL	whole plasma	NULL	NULL	NULL	NULL	gw60_circulation_99_2_237_s_139	9892589	44  45  Aggregated but not soluble native CRP selectively binds LDL and VLDL from whole plasma and, as we have previously proposed, could thereby participate in their atherogenic accumulation.	bind
55951	4	8225	6	13	NULL	NULL	NULL	CRP	GP	soluble;;native	does not bind					VLDL	GP				NULL	whole plasma	NULL	NULL	NULL	NULL	gw60_circulation_99_2_237_s_139	9892589	44  45  Aggregated but not soluble native CRP selectively binds LDL and VLDL from whole plasma and, as we have previously proposed, could thereby participate in their atherogenic accumulation.	bind
33220	1	8225	7	NULL	NULL	0	NULL	CRP	NULL	Aggregated	binds	NULL	selectively			LDL	NULL				NULL	whole plasma	0	NULL	NULL	NULL	gw60_circulation_99_2_237_s_139	9892589	44  45  Aggregated but not soluble native CRP selectively binds LDL and VLDL from whole plasma and, as we have previously proposed, could thereby participate in their atherogenic accumulation.	bind
33222	2	8225	7	NULL	NULL	0	NULL	CRP	NULL	Aggregated	binds	NULL	selectively			VLDL	NULL				NULL	whole plasma	0	NULL	NULL	NULL	gw60_circulation_99_2_237_s_139	9892589	44  45  Aggregated but not soluble native CRP selectively binds LDL and VLDL from whole plasma and, as we have previously proposed, could thereby participate in their atherogenic accumulation.	bind
33225	3	8225	7	NULL	NULL	0	NULL	CRP	NULL	soluble native	does not bind	NULL				LDL	NULL				NULL	whole plasma	NULL	NULL	NULL	NULL	gw60_circulation_99_2_237_s_139	9892589	44  45  Aggregated but not soluble native CRP selectively binds LDL and VLDL from whole plasma and, as we have previously proposed, could thereby participate in their atherogenic accumulation.	bind
33232	4	8225	7	NULL	NULL	0	NULL	CRP	NULL	soluble native	does not bind	NULL				VLDL	NULL				NULL	whole plasma	0	NULL	NULL	NULL	gw60_circulation_99_2_237_s_139	9892589	44  45  Aggregated but not soluble native CRP selectively binds LDL and VLDL from whole plasma and, as we have previously proposed, could thereby participate in their atherogenic accumulation.	bind
27291	1	8226	6	13	NULL	NULL	NULL	Caveolin-1	GP		interact		selectively			H-Ras	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_3_363_s_41	8781470	44  45  Caveolin-1 has also been shown to interact selectively with wild-type H-Ras but not with a mutationally activated soluble H-Ras, suggesting that caveolins may facilitate the binding of specific G proteins depending on their activation state.	bind
27292	2	8226	6	13	NULL	NULL	NULL	Caveolin-1	GP		does not interact with					H-Ras	GP	mutationally activated;;soluble			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_3_363_s_41	8781470	44  45  Caveolin-1 has also been shown to interact selectively with wild-type H-Ras but not with a mutationally activated soluble H-Ras, suggesting that caveolins may facilitate the binding of specific G proteins depending on their activation state.	bind
27293	3	8226	6	13	NULL	NULL	NULL	caveolins	GP		facilitate		may			G proteins	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_3_363_s_41	8781470	44  45  Caveolin-1 has also been shown to interact selectively with wild-type H-Ras but not with a mutationally activated soluble H-Ras, suggesting that caveolins may facilitate the binding of specific G proteins depending on their activation state.	bind
55952	4	8226	6	13	NULL	NULL	NULL	statement 3	Process		depends on					G proteins	GP	activation state of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_3_363_s_41	8781470	44  45  Caveolin-1 has also been shown to interact selectively with wild-type H-Ras but not with a mutationally activated soluble H-Ras, suggesting that caveolins may facilitate the binding of specific G proteins depending on their activation state.	bind
33243	1	8226	7	NULL	NULL	0	NULL	caveolin-1 	NULL		interacts with	NULL	selectively			H-Ras	NULL	wild-type			NULL		0	NULL	NULL	NULL	gw60_circulationres_79_3_363_s_41	8781470	44  45  Caveolin-1 has also been shown to interact selectively with wild-type H-Ras but not with a mutationally activated soluble H-Ras, suggesting that caveolins may facilitate the binding of specific G proteins depending on their activation state.	bind
33246	2	8226	7	10	NULL	0	NULL	caveolin-1			does not interact with					H-Ras		mutationally activated;;soluble			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_3_363_s_41	8781470	44  45  Caveolin-1 has also been shown to interact selectively with wild-type H-Ras but not with a mutationally activated soluble H-Ras, suggesting that caveolins may facilitate the binding of specific G proteins depending on their activation state.	bind
33248	3	8226	7	10	NULL	0	NULL	caveolins			facilitate		may			G proteins		binding of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_3_363_s_41	8781470	44  45  Caveolin-1 has also been shown to interact selectively with wild-type H-Ras but not with a mutationally activated soluble H-Ras, suggesting that caveolins may facilitate the binding of specific G proteins depending on their activation state.	bind
33249	4	8226	7	NULL	NULL	0	NULL	statement 3	NULL		depends on	NULL				G proteins	NULL	activation state of			NULL		0	NULL	NULL	NULL	gw60_circulationres_79_3_363_s_41	8781470	44  45  Caveolin-1 has also been shown to interact selectively with wild-type H-Ras but not with a mutationally activated soluble H-Ras, suggesting that caveolins may facilitate the binding of specific G proteins depending on their activation state.	bind
27294	1	8227	6	13	NULL	NULL	NULL	Neuropilin-1	GP		plays a role in					developing embryo	Organism				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_14_1887_s_159	11294808	44  Neuropilin-1 mutant mice were shown to exhibit various types of vascular defects, indicating a crucial role for this receptor in the developing embryo 45 ; still, the physiological consequences of VEGF binding to neuropilin receptors are yet to be fully explored.	bind
27295	2	8227	6	13	NULL	NULL	NULL	VEGF	GP		bind					neuropilin receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_14_1887_s_159	11294808	44  Neuropilin-1 mutant mice were shown to exhibit various types of vascular defects, indicating a crucial role for this receptor in the developing embryo 45 ; still, the physiological consequences of VEGF binding to neuropilin receptors are yet to be fully explored.	bind
27296	3	8227	6	13	NULL	NULL	NULL	Neuropilin-1	GP	mutant;;mice	exhibit					vascular defects	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_14_1887_s_159	11294808	44  Neuropilin-1 mutant mice were shown to exhibit various types of vascular defects, indicating a crucial role for this receptor in the developing embryo 45 ; still, the physiological consequences of VEGF binding to neuropilin receptors are yet to be fully explored.	bind
33250	1	8227	7	10	NULL	0	NULL	Neuropilin-1		mice;;mutant 	exhibit					vascular defects					NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_14_1887_s_159	11294808	44  Neuropilin-1 mutant mice were shown to exhibit various types of vascular defects, indicating a crucial role for this receptor in the developing embryo 45 ; still, the physiological consequences of VEGF binding to neuropilin receptors are yet to be fully explored.	bind
33251	2	8227	7	NULL	NULL	0	NULL	statement 1	NULL		indicate	NULL				Neuropilin receptor	NULL	crucial role of			NULL	developing embryo	NULL	NULL	NULL	NULL	gw60_circulation_103_14_1887_s_159	11294808	44  Neuropilin-1 mutant mice were shown to exhibit various types of vascular defects, indicating a crucial role for this receptor in the developing embryo 45 ; still, the physiological consequences of VEGF binding to neuropilin receptors are yet to be fully explored.	bind
33252	3	8227	7	NULL	NULL	0	NULL	VEGF	NULL		binds to	NULL				neuropilin receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_14_1887_s_159	11294808	44  Neuropilin-1 mutant mice were shown to exhibit various types of vascular defects, indicating a crucial role for this receptor in the developing embryo 45 ; still, the physiological consequences of VEGF binding to neuropilin receptors are yet to be fully explored.	bind
27297	1	8228	6	13	NULL	NULL	NULL	Sp1	GP		bind					TF	GP	human		GC box in promoter	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_2_365_s_214	9081693	44 45  In our studies, EMSAs identified binding of Sp1 to five distinct GC boxes in the human TF promoter.	bind
33253	1	8228	7	NULL	NULL	0	NULL	Sp1	NULL		bind	NULL				TF	NULL	human		GC boxes in the promoter	NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_2_365_s_214	9081693	44 45  In our studies, EMSAs identified binding of Sp1 to five distinct GC boxes in the human TF promoter.	bind
27298	1	8229	6	13	NULL	NULL	NULL	ATIII	GP		bind					thrombin	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_4_495_s_171	7749861	44 45 46 47 48  Conard et al 45  have indicated that plasma ATIII levels can be underestimated when obtained by the active-site titration technique with thrombin in the presence of heparin because heparin can interfere with the stoichiometry of thrombin binding by ATIII.	bind
27299	2	8229	6	13	NULL	NULL	NULL	heparin	Chemical		interfere with					statement 1	Process	stoichiometry of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_4_495_s_171	7749861	44 45 46 47 48  Conard et al 45  have indicated that plasma ATIII levels can be underestimated when obtained by the active-site titration technique with thrombin in the presence of heparin because heparin can interfere with the stoichiometry of thrombin binding by ATIII.	bind
33254	1	8229	7	NULL	NULL	0	NULL	ATIII	NULL		bind	NULL				thrombin	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_4_495_s_171	7749861	44 45 46 47 48  Conard et al 45  have indicated that plasma ATIII levels can be underestimated when obtained by the active-site titration technique with thrombin in the presence of heparin because heparin can interfere with the stoichiometry of thrombin binding by ATIII.	bind
33255	2	8229	7	NULL	NULL	0	NULL	heparin	NULL		interferes with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_4_495_s_171	7749861	44 45 46 47 48  Conard et al 45  have indicated that plasma ATIII levels can be underestimated when obtained by the active-site titration technique with thrombin in the presence of heparin because heparin can interfere with the stoichiometry of thrombin binding by ATIII.	bind
27555	1	8230	6	13	NULL	NULL	NULL	HDL3 containing apoA-I	GP		exhibits					CETP activity	GP	plasma			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_213_s_210	8620335	44 54 The majority of the plasma CETP activity has been located in HDL3, 43  with lipoproteins containing apoA-I but no apoA-II, 45  or in HDL3, VHDL, and to a lesser extent HDL2, but not in VLDL or LDL. 53  Others, however, have detected binding of CETP to both Sepharose-bound VLDL and LDL, in addition to HDL. 44 54  CETP has been observed in rabbits to be associated with small HDL particles.	bind
27556	2	8230	6	13	NULL	NULL	NULL	HDL3 containing apoA-II	GP		does not exhibit					CETP activity	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_213_s_210	8620335	44 54 The majority of the plasma CETP activity has been located in HDL3, 43  with lipoproteins containing apoA-I but no apoA-II, 45  or in HDL3, VHDL, and to a lesser extent HDL2, but not in VLDL or LDL. 53  Others, however, have detected binding of CETP to both Sepharose-bound VLDL and LDL, in addition to HDL. 44 54  CETP has been observed in rabbits to be associated with small HDL particles.	bind
27557	3	8230	6	13	NULL	NULL	NULL	HDL2	GP		exhibits					CETP activity	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_213_s_210	8620335	44 54 The majority of the plasma CETP activity has been located in HDL3, 43  with lipoproteins containing apoA-I but no apoA-II, 45  or in HDL3, VHDL, and to a lesser extent HDL2, but not in VLDL or LDL. 53  Others, however, have detected binding of CETP to both Sepharose-bound VLDL and LDL, in addition to HDL. 44 54  CETP has been observed in rabbits to be associated with small HDL particles.	bind
27558	4	8230	6	13	NULL	NULL	NULL	VLDL	GP		does not exhibit					CETP activity	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_213_s_210	8620335	44 54 The majority of the plasma CETP activity has been located in HDL3, 43  with lipoproteins containing apoA-I but no apoA-II, 45  or in HDL3, VHDL, and to a lesser extent HDL2, but not in VLDL or LDL. 53  Others, however, have detected binding of CETP to both Sepharose-bound VLDL and LDL, in addition to HDL. 44 54  CETP has been observed in rabbits to be associated with small HDL particles.	bind
27559	5	8230	6	13	NULL	NULL	NULL	LDL	GP		does not exhibit					CETP activity	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_213_s_210	8620335	44 54 The majority of the plasma CETP activity has been located in HDL3, 43  with lipoproteins containing apoA-I but no apoA-II, 45  or in HDL3, VHDL, and to a lesser extent HDL2, but not in VLDL or LDL. 53  Others, however, have detected binding of CETP to both Sepharose-bound VLDL and LDL, in addition to HDL. 44 54  CETP has been observed in rabbits to be associated with small HDL particles.	bind
27560	6	8230	6	13	NULL	NULL	NULL	CETP	GP		associates with					HDL particles	GP	small			NULL	rabbits	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_213_s_210	8620335	44 54 The majority of the plasma CETP activity has been located in HDL3, 43  with lipoproteins containing apoA-I but no apoA-II, 45  or in HDL3, VHDL, and to a lesser extent HDL2, but not in VLDL or LDL. 53  Others, however, have detected binding of CETP to both Sepharose-bound VLDL and LDL, in addition to HDL. 44 54  CETP has been observed in rabbits to be associated with small HDL particles.	bind
33256	1	8230	7	NULL	NULL	0	NULL	CETP activity	NULL	plasma	is located in	NULL				HDL3	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_213_s_210	8620335	44 54 The majority of the plasma CETP activity has been located in HDL3, 43  with lipoproteins containing apoA-I but no apoA-II, 45  or in HDL3, VHDL, and to a lesser extent HDL2, but not in VLDL or LDL. 53  Others, however, have detected binding of CETP to both Sepharose-bound VLDL and LDL, in addition to HDL. 44 54  CETP has been observed in rabbits to be associated with small HDL particles.	bind
33257	2	8230	7	NULL	NULL	0	NULL	HDL3	NULL		contains	NULL				apoA-I	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_213_s_210	8620335	44 54 The majority of the plasma CETP activity has been located in HDL3, 43  with lipoproteins containing apoA-I but no apoA-II, 45  or in HDL3, VHDL, and to a lesser extent HDL2, but not in VLDL or LDL. 53  Others, however, have detected binding of CETP to both Sepharose-bound VLDL and LDL, in addition to HDL. 44 54  CETP has been observed in rabbits to be associated with small HDL particles.	bind
33260	3	8230	7	NULL	NULL	0	NULL	HDL3	NULL		does not contain	NULL				apoA-II	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_213_s_210	8620335	44 54 The majority of the plasma CETP activity has been located in HDL3, 43  with lipoproteins containing apoA-I but no apoA-II, 45  or in HDL3, VHDL, and to a lesser extent HDL2, but not in VLDL or LDL. 53  Others, however, have detected binding of CETP to both Sepharose-bound VLDL and LDL, in addition to HDL. 44 54  CETP has been observed in rabbits to be associated with small HDL particles.	bind
33262	4	8230	7	NULL	NULL	0	NULL	CETP activity	NULL	plasma	is located in	NULL				VHDL	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_213_s_210	8620335	44 54 The majority of the plasma CETP activity has been located in HDL3, 43  with lipoproteins containing apoA-I but no apoA-II, 45  or in HDL3, VHDL, and to a lesser extent HDL2, but not in VLDL or LDL. 53  Others, however, have detected binding of CETP to both Sepharose-bound VLDL and LDL, in addition to HDL. 44 54  CETP has been observed in rabbits to be associated with small HDL particles.	bind
33263	5	8230	7	NULL	NULL	0	NULL	CETP activity	NULL	plasma	is located in	NULL	less extent			HDL2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_213_s_210	8620335	44 54 The majority of the plasma CETP activity has been located in HDL3, 43  with lipoproteins containing apoA-I but no apoA-II, 45  or in HDL3, VHDL, and to a lesser extent HDL2, but not in VLDL or LDL. 53  Others, however, have detected binding of CETP to both Sepharose-bound VLDL and LDL, in addition to HDL. 44 54  CETP has been observed in rabbits to be associated with small HDL particles.	bind
33264	6	8230	7	NULL	NULL	0	NULL	CETP activity	NULL		is not present in	NULL				VLDL	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_213_s_210	8620335	44 54 The majority of the plasma CETP activity has been located in HDL3, 43  with lipoproteins containing apoA-I but no apoA-II, 45  or in HDL3, VHDL, and to a lesser extent HDL2, but not in VLDL or LDL. 53  Others, however, have detected binding of CETP to both Sepharose-bound VLDL and LDL, in addition to HDL. 44 54  CETP has been observed in rabbits to be associated with small HDL particles.	bind
33265	7	8230	7	NULL	NULL	0	NULL	CETP activity	NULL		is not present in	NULL				LDL	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_213_s_210	8620335	44 54 The majority of the plasma CETP activity has been located in HDL3, 43  with lipoproteins containing apoA-I but no apoA-II, 45  or in HDL3, VHDL, and to a lesser extent HDL2, but not in VLDL or LDL. 53  Others, however, have detected binding of CETP to both Sepharose-bound VLDL and LDL, in addition to HDL. 44 54  CETP has been observed in rabbits to be associated with small HDL particles.	bind
33266	8	8230	7	NULL	NULL	0	NULL	CETP	NULL		bind	NULL				Sepharose-bound VLDL	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_213_s_210	8620335	44 54 The majority of the plasma CETP activity has been located in HDL3, 43  with lipoproteins containing apoA-I but no apoA-II, 45  or in HDL3, VHDL, and to a lesser extent HDL2, but not in VLDL or LDL. 53  Others, however, have detected binding of CETP to both Sepharose-bound VLDL and LDL, in addition to HDL. 44 54  CETP has been observed in rabbits to be associated with small HDL particles.	bind
33267	9	8230	7	NULL	NULL	0	NULL	CETP	NULL		bind	NULL				LDL	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_213_s_210	8620335	44 54 The majority of the plasma CETP activity has been located in HDL3, 43  with lipoproteins containing apoA-I but no apoA-II, 45  or in HDL3, VHDL, and to a lesser extent HDL2, but not in VLDL or LDL. 53  Others, however, have detected binding of CETP to both Sepharose-bound VLDL and LDL, in addition to HDL. 44 54  CETP has been observed in rabbits to be associated with small HDL particles.	bind
33269	10	8230	7	NULL	NULL	0	NULL	CETP	NULL		bind	NULL				HDL	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_213_s_210	8620335	44 54 The majority of the plasma CETP activity has been located in HDL3, 43  with lipoproteins containing apoA-I but no apoA-II, 45  or in HDL3, VHDL, and to a lesser extent HDL2, but not in VLDL or LDL. 53  Others, however, have detected binding of CETP to both Sepharose-bound VLDL and LDL, in addition to HDL. 44 54  CETP has been observed in rabbits to be associated with small HDL particles.	bind
33270	11	8230	7	NULL	NULL	0	NULL	CETP	NULL		 associate with	NULL				small HDL particles	NULL				NULL	rabbits	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_213_s_210	8620335	44 54 The majority of the plasma CETP activity has been located in HDL3, 43  with lipoproteins containing apoA-I but no apoA-II, 45  or in HDL3, VHDL, and to a lesser extent HDL2, but not in VLDL or LDL. 53  Others, however, have detected binding of CETP to both Sepharose-bound VLDL and LDL, in addition to HDL. 44 54  CETP has been observed in rabbits to be associated with small HDL particles.	bind
27300	1	8231	6	13	NULL	NULL	NULL	Cu2+	Chemical		bind					PrP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_6795_s_50	12454014	44 and  46), and the number of Cu2+ ions binding to PrP is in dispute.	bind
33300	1	8231	7	NULL	NULL	0	NULL	Cu2+ ions	NULL		bind	NULL				PrP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_9_6795_s_50	12454014	44 and  46), and the number of Cu2+ ions binding to PrP is in dispute.	bind
27301	1	8232	6	13	NULL	NULL	NULL	MGP	GP		bind					BMP2	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1423_s_126	16601233	44 MGP is a calcium-binding matrix protein that binds and inhibits BMP2 induction of ALP. 45 In addition, carboxylated MGP produced by VSMCs binds matrix elastin and inhibits calcification.	bind
27302	2	8232	6	13	NULL	NULL	NULL	BMP2	GP		induces					ALP	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1423_s_126	16601233	44 MGP is a calcium-binding matrix protein that binds and inhibits BMP2 induction of ALP. 45 In addition, carboxylated MGP produced by VSMCs binds matrix elastin and inhibits calcification.	bind
27303	3	8232	6	13	NULL	NULL	NULL	MGP	GP		inhibits					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1423_s_126	16601233	44 MGP is a calcium-binding matrix protein that binds and inhibits BMP2 induction of ALP. 45 In addition, carboxylated MGP produced by VSMCs binds matrix elastin and inhibits calcification.	bind
27304	4	8232	6	13	NULL	NULL	NULL	MGP	GP		is a type of					calcium-binding matrix protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1423_s_126	16601233	44 MGP is a calcium-binding matrix protein that binds and inhibits BMP2 induction of ALP. 45 In addition, carboxylated MGP produced by VSMCs binds matrix elastin and inhibits calcification.	bind
27305	5	8232	6	13	NULL	NULL	NULL	VSMC	Cell		produce					MGP	GP	carboxylated			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1423_s_126	16601233	44 MGP is a calcium-binding matrix protein that binds and inhibits BMP2 induction of ALP. 45 In addition, carboxylated MGP produced by VSMCs binds matrix elastin and inhibits calcification.	bind
27306	6	8232	6	13	NULL	NULL	NULL	MGP	GP	carboxylated	bind					matrix elastin	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1423_s_126	16601233	44 MGP is a calcium-binding matrix protein that binds and inhibits BMP2 induction of ALP. 45 In addition, carboxylated MGP produced by VSMCs binds matrix elastin and inhibits calcification.	bind
27307	7	8232	6	13	NULL	NULL	NULL	statement 6	Process		inhibits					calcification	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1423_s_126	16601233	44 MGP is a calcium-binding matrix protein that binds and inhibits BMP2 induction of ALP. 45 In addition, carboxylated MGP produced by VSMCs binds matrix elastin and inhibits calcification.	bind
33301	1	8232	7	NULL	NULL	0	NULL	 MGP	NULL		is a type of	NULL				calcium-binding matrix protein	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1423_s_126	16601233	44 MGP is a calcium-binding matrix protein that binds and inhibits BMP2 induction of ALP. 45 In addition, carboxylated MGP produced by VSMCs binds matrix elastin and inhibits calcification.	bind
33302	2	8232	7	NULL	NULL	0	NULL	MGP	NULL		binds	NULL				BMP2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1423_s_126	16601233	44 MGP is a calcium-binding matrix protein that binds and inhibits BMP2 induction of ALP. 45 In addition, carboxylated MGP produced by VSMCs binds matrix elastin and inhibits calcification.	bind
33303	3	8232	7	NULL	NULL	0	NULL	BMP2	NULL		induce	NULL				ALP	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1423_s_126	16601233	44 MGP is a calcium-binding matrix protein that binds and inhibits BMP2 induction of ALP. 45 In addition, carboxylated MGP produced by VSMCs binds matrix elastin and inhibits calcification.	bind
33304	4	8232	7	NULL	NULL	0	NULL	statement 2	NULL		inhibits	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1423_s_126	16601233	44 MGP is a calcium-binding matrix protein that binds and inhibits BMP2 induction of ALP. 45 In addition, carboxylated MGP produced by VSMCs binds matrix elastin and inhibits calcification.	bind
33305	5	8232	7	10	NULL	0	NULL	VSMCs	NULL		produce	NULL				MGP	NULL	carboxylated			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1423_s_126	16601233	44 MGP is a calcium-binding matrix protein that binds and inhibits BMP2 induction of ALP. 45 In addition, carboxylated MGP produced by VSMCs binds matrix elastin and inhibits calcification.	bind
33306	6	8232	7	10	NULL	0	NULL	MGP	NULL	carboxylated	binds	NULL				matrix elastin	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1423_s_126	16601233	44 MGP is a calcium-binding matrix protein that binds and inhibits BMP2 induction of ALP. 45 In addition, carboxylated MGP produced by VSMCs binds matrix elastin and inhibits calcification.	bind
33307	7	8232	7	NULL	NULL	0	NULL	statement 6	NULL		inhibits	NULL				calcification	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1423_s_126	16601233	44 MGP is a calcium-binding matrix protein that binds and inhibits BMP2 induction of ALP. 45 In addition, carboxylated MGP produced by VSMCs binds matrix elastin and inhibits calcification.	bind
27308	1	8233	6	13	NULL	NULL	NULL	heparin	Chemical		bind					growth factors	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_9_937_s_220	16195480	44 Though heparin binding to growth factors may be involved in the inhibition of PASMC proliferation, this is not the only mechanism.	bind
27309	2	8233	6	13	NULL	NULL	NULL	statement 1	Process		is involved in					PASMC	Cell	inhibiton of;;proliferation of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_9_937_s_220	16195480	44 Though heparin binding to growth factors may be involved in the inhibition of PASMC proliferation, this is not the only mechanism.	bind
33308	1	8233	7	NULL	NULL	0	NULL	heparin	NULL		bind	NULL				growth factors	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_9_937_s_220	16195480	44 Though heparin binding to growth factors may be involved in the inhibition of PASMC proliferation, this is not the only mechanism.	bind
33309	2	8233	7	10	NULL	0	NULL	statement 1	NULL		be involved in	NULL	may			PASMC 	NULL	inhibition of;;proliferation of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_9_937_s_220	16195480	44 Though heparin binding to growth factors may be involved in the inhibition of PASMC proliferation, this is not the only mechanism.	bind
27310	1	8234	6	13	NULL	NULL	NULL	TIMP-2	GP		bind					proMMP-2	GP		hemopexin domain		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_8_827_s_118	12730128	44 TIMP-2 binds to the hemopexin domain of proMMP-2.	bind
33310	1	8234	7	NULL	NULL	0	NULL	TIMP-2 	NULL		binds to	NULL				proMMP-2	NULL		hemopexin domain		NULL		0	NULL	NULL	NULL	gw70_circulationres_92_8_827_s_118	12730128	44 TIMP-2 binds to the hemopexin domain of proMMP-2.	bind
27311	1	8235	6	13	NULL	NULL	NULL	VEGF	GP		bind					VEGF receptor 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1143_s_113	12676799	44 We also discovered that the weak arteriogenic effects of chronically infused VEGF A is caused by the monocyte attractant effect of VEGF that binds to the VEGF receptor 1, which is exclusively present on monocytes.	bind
27312	2	8235	6	13	NULL	NULL	NULL	VEGF receptor	GP		is present on		exclusively			monocytes	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1143_s_113	12676799	44 We also discovered that the weak arteriogenic effects of chronically infused VEGF A is caused by the monocyte attractant effect of VEGF that binds to the VEGF receptor 1, which is exclusively present on monocytes.	bind
27313	3	8235	6	13	NULL	NULL	NULL	VEGF 	GP		exhibits					monocyte attractant effect	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1143_s_113	12676799	44 We also discovered that the weak arteriogenic effects of chronically infused VEGF A is caused by the monocyte attractant effect of VEGF that binds to the VEGF receptor 1, which is exclusively present on monocytes.	bind
27314	4	8235	6	13	NULL	NULL	NULL	VEGF A	GP	weak arteriogenic effects of	is caused by					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1143_s_113	12676799	44 We also discovered that the weak arteriogenic effects of chronically infused VEGF A is caused by the monocyte attractant effect of VEGF that binds to the VEGF receptor 1, which is exclusively present on monocytes.	bind
33311	1	8235	7	NULL	NULL	0	NULL	VEGF 	NULL		binds to	NULL				VEGF receptor 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1143_s_113	12676799	44 We also discovered that the weak arteriogenic effects of chronically infused VEGF A is caused by the monocyte attractant effect of VEGF that binds to the VEGF receptor 1, which is exclusively present on monocytes.	bind
33312	2	8235	7	NULL	NULL	0	NULL	VEGF	NULL		attract	NULL				monocyte	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1143_s_113	12676799	44 We also discovered that the weak arteriogenic effects of chronically infused VEGF A is caused by the monocyte attractant effect of VEGF that binds to the VEGF receptor 1, which is exclusively present on monocytes.	bind
33313	3	8235	7	NULL	NULL	0	NULL	statement 2	NULL		cause	NULL				VEGF A	NULL	weak arteriogenic effects of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1143_s_113	12676799	44 We also discovered that the weak arteriogenic effects of chronically infused VEGF A is caused by the monocyte attractant effect of VEGF that binds to the VEGF receptor 1, which is exclusively present on monocytes.	bind
33314	4	8235	7	NULL	NULL	0	NULL	VEGF receptor 1	NULL		 present in	NULL	exclusively			monocytes	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1143_s_113	12676799	44 We also discovered that the weak arteriogenic effects of chronically infused VEGF A is caused by the monocyte attractant effect of VEGF that binds to the VEGF receptor 1, which is exclusively present on monocytes.	bind
27315	1	8236	6	13	NULL	NULL	NULL	fibronectin	GP		bind					collagen	GP	native			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_5_1489_s_153	10793060	44, 105  Although fibronectin does bind native collagens, it shows a markedly increased affinity for denatured collagen.	bind
27316	2	8236	6	13	NULL	NULL	NULL	fibronectin	GP		bind					collagen	GP	denatured			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_5_1489_s_153	10793060	44, 105  Although fibronectin does bind native collagens, it shows a markedly increased affinity for denatured collagen.	bind
46708	3	8236	6	13	NULL	NULL	NULL	statement 2	Process	affinity of	is higher than					statement 1	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_5_1489_s_153	10793060	44, 105  Although fibronectin does bind native collagens, it shows a markedly increased affinity for denatured collagen.	bind
33315	1	8236	7	NULL	NULL	0	NULL	fibronectin	NULL		bind	NULL				collagen	NULL	native			NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_5_1489_s_153	10793060	44, 105  Although fibronectin does bind native collagens, it shows a markedly increased affinity for denatured collagen.	bind
33316	2	8236	7	NULL	NULL	0	NULL	fibronectin	NULL		bind	NULL				collagen	NULL	denatured			NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_5_1489_s_153	10793060	44, 105  Although fibronectin does bind native collagens, it shows a markedly increased affinity for denatured collagen.	bind
33317	3	8236	7	NULL	NULL	0	NULL	statement 2	NULL	affinity of	is higher than	NULL				statement 1	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_5_1489_s_153	10793060	44, 105  Although fibronectin does bind native collagens, it shows a markedly increased affinity for denatured collagen.	bind
27317	1	8237	6	13	NULL	NULL	NULL	IGF-1	GP		bind					IGF-1R	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_94	14604834	44,45  However, proteolysis or polymerization of IGFBPs or binding to extracellular matrix results in reduction or loss of IGF-1 binding to IGFBPs, thus increasing the binding of IGF-1 to IGF-1R and the activity of IGF-1.	bind
27318	2	8237	6	13	NULL	NULL	NULL	IGF-1	GP		bind					IGFBP	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_94	14604834	44,45  However, proteolysis or polymerization of IGFBPs or binding to extracellular matrix results in reduction or loss of IGF-1 binding to IGFBPs, thus increasing the binding of IGF-1 to IGF-1R and the activity of IGF-1.	bind
27319	3	8237	6	13	NULL	NULL	NULL	IGFBP	GP		bind					extracellular matrix	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_94	14604834	44,45  However, proteolysis or polymerization of IGFBPs or binding to extracellular matrix results in reduction or loss of IGF-1 binding to IGFBPs, thus increasing the binding of IGF-1 to IGF-1R and the activity of IGF-1.	bind
27320	4	8237	6	13	NULL	NULL	NULL	IGFBP	GP	proteolysis of	results in					statement 2	Process	loss of 			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_94	14604834	44,45  However, proteolysis or polymerization of IGFBPs or binding to extracellular matrix results in reduction or loss of IGF-1 binding to IGFBPs, thus increasing the binding of IGF-1 to IGF-1R and the activity of IGF-1.	bind
27321	5	8237	6	13	NULL	NULL	NULL	IGFBP	GP	polymerization of 	results in					statement 2	Process	loss of 			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_94	14604834	44,45  However, proteolysis or polymerization of IGFBPs or binding to extracellular matrix results in reduction or loss of IGF-1 binding to IGFBPs, thus increasing the binding of IGF-1 to IGF-1R and the activity of IGF-1.	bind
27322	6	8237	6	13	NULL	NULL	NULL	IGFBP	GP	proteolysis of	increases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_94	14604834	44,45  However, proteolysis or polymerization of IGFBPs or binding to extracellular matrix results in reduction or loss of IGF-1 binding to IGFBPs, thus increasing the binding of IGF-1 to IGF-1R and the activity of IGF-1.	bind
27323	7	8237	6	13	NULL	NULL	NULL	IGFBP	GP	polymerization of	increases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_94	14604834	44,45  However, proteolysis or polymerization of IGFBPs or binding to extracellular matrix results in reduction or loss of IGF-1 binding to IGFBPs, thus increasing the binding of IGF-1 to IGF-1R and the activity of IGF-1.	bind
27324	8	8237	6	13	NULL	NULL	NULL	IGFBP	GP	proteolysis of	increases					IGF-1	GP	activity of 			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_94	14604834	44,45  However, proteolysis or polymerization of IGFBPs or binding to extracellular matrix results in reduction or loss of IGF-1 binding to IGFBPs, thus increasing the binding of IGF-1 to IGF-1R and the activity of IGF-1.	bind
27325	9	8237	6	13	NULL	NULL	NULL	IGFBP	GP	polymerization of	increases					IGF-1	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_94	14604834	44,45  However, proteolysis or polymerization of IGFBPs or binding to extracellular matrix results in reduction or loss of IGF-1 binding to IGFBPs, thus increasing the binding of IGF-1 to IGF-1R and the activity of IGF-1.	bind
33318	1	8237	7	NULL	NULL	0	NULL	IGFBPs	NULL		undergoes	NULL				polymerization 	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_94	14604834	44,45  However, proteolysis or polymerization of IGFBPs or binding to extracellular matrix results in reduction or loss of IGF-1 binding to IGFBPs, thus increasing the binding of IGF-1 to IGF-1R and the activity of IGF-1.	bind
33319	2	8237	7	NULL	NULL	0	NULL	IGFBPs	NULL		undergoes	NULL				proteolysis	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_94	14604834	44,45  However, proteolysis or polymerization of IGFBPs or binding to extracellular matrix results in reduction or loss of IGF-1 binding to IGFBPs, thus increasing the binding of IGF-1 to IGF-1R and the activity of IGF-1.	bind
33320	3	8237	7	NULL	NULL	0	NULL	IGFBPs	NULL		bind	NULL				extracellular matrix	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_94	14604834	44,45  However, proteolysis or polymerization of IGFBPs or binding to extracellular matrix results in reduction or loss of IGF-1 binding to IGFBPs, thus increasing the binding of IGF-1 to IGF-1R and the activity of IGF-1.	bind
33321	4	8237	7	NULL	NULL	0	NULL	IGF-1	NULL		bind	NULL				IGFBPs	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_94	14604834	44,45  However, proteolysis or polymerization of IGFBPs or binding to extracellular matrix results in reduction or loss of IGF-1 binding to IGFBPs, thus increasing the binding of IGF-1 to IGF-1R and the activity of IGF-1.	bind
33322	5	8237	7	NULL	NULL	0	NULL	statement 1	NULL		reduce	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_94	14604834	44,45  However, proteolysis or polymerization of IGFBPs or binding to extracellular matrix results in reduction or loss of IGF-1 binding to IGFBPs, thus increasing the binding of IGF-1 to IGF-1R and the activity of IGF-1.	bind
33323	6	8237	7	NULL	NULL	0	NULL	statement 2	NULL		reduce	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_94	14604834	44,45  However, proteolysis or polymerization of IGFBPs or binding to extracellular matrix results in reduction or loss of IGF-1 binding to IGFBPs, thus increasing the binding of IGF-1 to IGF-1R and the activity of IGF-1.	bind
33324	7	8237	7	NULL	NULL	0	NULL	statement 3	NULL		reduce	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_94	14604834	44,45  However, proteolysis or polymerization of IGFBPs or binding to extracellular matrix results in reduction or loss of IGF-1 binding to IGFBPs, thus increasing the binding of IGF-1 to IGF-1R and the activity of IGF-1.	bind
33325	8	8237	7	NULL	NULL	0	NULL	statement 1	NULL		results in	NULL				statement 4	NULL	loss of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_94	14604834	44,45  However, proteolysis or polymerization of IGFBPs or binding to extracellular matrix results in reduction or loss of IGF-1 binding to IGFBPs, thus increasing the binding of IGF-1 to IGF-1R and the activity of IGF-1.	bind
33326	9	8237	7	NULL	NULL	0	NULL	statement 2	NULL		results in	NULL				statement 4	NULL	loss of 			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_94	14604834	44,45  However, proteolysis or polymerization of IGFBPs or binding to extracellular matrix results in reduction or loss of IGF-1 binding to IGFBPs, thus increasing the binding of IGF-1 to IGF-1R and the activity of IGF-1.	bind
33327	10	8237	7	NULL	NULL	0	NULL	statement 3	NULL		results in	NULL				statement 4	NULL	loss of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_94	14604834	44,45  However, proteolysis or polymerization of IGFBPs or binding to extracellular matrix results in reduction or loss of IGF-1 binding to IGFBPs, thus increasing the binding of IGF-1 to IGF-1R and the activity of IGF-1.	bind
33328	11	8237	7	NULL	NULL	0	NULL	statement 5	NULL		is an alternative to	NULL				statement 8	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_94	14604834	44,45  However, proteolysis or polymerization of IGFBPs or binding to extracellular matrix results in reduction or loss of IGF-1 binding to IGFBPs, thus increasing the binding of IGF-1 to IGF-1R and the activity of IGF-1.	bind
33329	12	8237	7	NULL	NULL	0	NULL	statement 6	NULL		is an alternative to	NULL				statement 9	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_94	14604834	44,45  However, proteolysis or polymerization of IGFBPs or binding to extracellular matrix results in reduction or loss of IGF-1 binding to IGFBPs, thus increasing the binding of IGF-1 to IGF-1R and the activity of IGF-1.	bind
33330	13	8237	7	NULL	NULL	0	NULL	statement 7	NULL		is an alternative to	NULL				statement 10	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_94	14604834	44,45  However, proteolysis or polymerization of IGFBPs or binding to extracellular matrix results in reduction or loss of IGF-1 binding to IGFBPs, thus increasing the binding of IGF-1 to IGF-1R and the activity of IGF-1.	bind
33331	14	8237	7	NULL	NULL	0	NULL	IGF-1	NULL		bind	NULL				IGF-1R 	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_94	14604834	44,45  However, proteolysis or polymerization of IGFBPs or binding to extracellular matrix results in reduction or loss of IGF-1 binding to IGFBPs, thus increasing the binding of IGF-1 to IGF-1R and the activity of IGF-1.	bind
33332	15	8237	7	NULL	NULL	0	NULL	statement 11	NULL		increase	NULL				statement 14	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_94	14604834	44,45  However, proteolysis or polymerization of IGFBPs or binding to extracellular matrix results in reduction or loss of IGF-1 binding to IGFBPs, thus increasing the binding of IGF-1 to IGF-1R and the activity of IGF-1.	bind
33333	16	8237	7	NULL	NULL	0	NULL	statement 12	NULL		increase	NULL				statement 14	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_94	14604834	44,45  However, proteolysis or polymerization of IGFBPs or binding to extracellular matrix results in reduction or loss of IGF-1 binding to IGFBPs, thus increasing the binding of IGF-1 to IGF-1R and the activity of IGF-1.	bind
33334	17	8237	7	NULL	NULL	0	NULL	statement 13	NULL		increase	NULL				statement 14	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_94	14604834	44,45  However, proteolysis or polymerization of IGFBPs or binding to extracellular matrix results in reduction or loss of IGF-1 binding to IGFBPs, thus increasing the binding of IGF-1 to IGF-1R and the activity of IGF-1.	bind
33335	18	8237	7	NULL	NULL	0	NULL	statement 11	NULL		increase	NULL				IGF-1	NULL	activity of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_94	14604834	44,45  However, proteolysis or polymerization of IGFBPs or binding to extracellular matrix results in reduction or loss of IGF-1 binding to IGFBPs, thus increasing the binding of IGF-1 to IGF-1R and the activity of IGF-1.	bind
33336	19	8237	7	NULL	NULL	0	NULL	statement 12	NULL		increase	NULL				IGF-1	NULL	activity of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_94	14604834	44,45  However, proteolysis or polymerization of IGFBPs or binding to extracellular matrix results in reduction or loss of IGF-1 binding to IGFBPs, thus increasing the binding of IGF-1 to IGF-1R and the activity of IGF-1.	bind
33337	20	8237	7	NULL	NULL	0	NULL	statement 13	NULL		increase	NULL				IGF-1	NULL	activity of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_3_435_s_94	14604834	44,45  However, proteolysis or polymerization of IGFBPs or binding to extracellular matrix results in reduction or loss of IGF-1 binding to IGFBPs, thus increasing the binding of IGF-1 to IGF-1R and the activity of IGF-1.	bind
27326	1	8238	6	13	NULL	NULL	NULL	collagenase gene	GP		contains				promoter					TPA responsive unit	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1661_s_467	11292838	45       Gutman,A. and Wasylyk,B. (1990) The collagenase gene promoter contains a TPA and oncogene-responsive unit encompassing the PEA3 and AP-1 binding sites.	bind
27327	2	8238	6	13	NULL	NULL	NULL	collagenase gene	GP		contains				promoter					oncogene-responsive unit	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1661_s_467	11292838	45       Gutman,A. and Wasylyk,B. (1990) The collagenase gene promoter contains a TPA and oncogene-responsive unit encompassing the PEA3 and AP-1 binding sites.	bind
46709	3	8238	6	10	NULL	0	NULL		NULL		encompass	NULL			oncogene-responsive unit		NULL			AP-1 binding site	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1661_s_467	11292838	45       Gutman,A. and Wasylyk,B. (1990) The collagenase gene promoter contains a TPA and oncogene-responsive unit encompassing the PEA3 and AP-1 binding sites.	bind
46710	4	8238	6	10	NULL	0	NULL		NULL		encompass	NULL			TPA responsive unit		NULL			PEA3 binding site	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1661_s_467	11292838	45       Gutman,A. and Wasylyk,B. (1990) The collagenase gene promoter contains a TPA and oncogene-responsive unit encompassing the PEA3 and AP-1 binding sites.	bind
33338	1	8238	7	NULL	NULL	0	NULL	collagenase gene	NULL		contains	NULL			promoter		NULL			TPA responsive unit	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1661_s_467	11292838	45       Gutman,A. and Wasylyk,B. (1990) The collagenase gene promoter contains a TPA and oncogene-responsive unit encompassing the PEA3 and AP-1 binding sites.	bind
33339	2	8238	7	NULL	NULL	0	NULL	collagenase gene	NULL		contains	NULL			promoter		NULL			oncogene-responsive unit	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1661_s_467	11292838	45       Gutman,A. and Wasylyk,B. (1990) The collagenase gene promoter contains a TPA and oncogene-responsive unit encompassing the PEA3 and AP-1 binding sites.	bind
33340	3	8238	7	NULL	NULL	0	NULL		NULL		encompass	NULL			 TPA responsive unit		NULL			PEA3 binding site	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1661_s_467	11292838	45       Gutman,A. and Wasylyk,B. (1990) The collagenase gene promoter contains a TPA and oncogene-responsive unit encompassing the PEA3 and AP-1 binding sites.	bind
33341	4	8238	7	NULL	NULL	0	NULL		NULL		encompass	NULL			oncogene-responsive unit		NULL			AP-1 binding site	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1661_s_467	11292838	45       Gutman,A. and Wasylyk,B. (1990) The collagenase gene promoter contains a TPA and oncogene-responsive unit encompassing the PEA3 and AP-1 binding sites.	bind
27328	1	8239	6	13	NULL	NULL	NULL	GAL4	GP		bind		facilitated			nucleosomal template	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_17_3520_s_420	11522821	45       Taylor,I.C.A., Workman,J.L., Schuetz,T.J. and Kingston,R.E. (1991) Facilitated binding of GAL4 and heat shock factor to nucleosomal templates: differential function of DNA binding domains.	bind
27329	2	8239	6	13	NULL	NULL	NULL	heat shock factor	GP		bind		facilitated			nucleosomal template	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_17_3520_s_420	11522821	45       Taylor,I.C.A., Workman,J.L., Schuetz,T.J. and Kingston,R.E. (1991) Facilitated binding of GAL4 and heat shock factor to nucleosomal templates: differential function of DNA binding domains.	bind
33342	1	8239	7	NULL	NULL	0	NULL	GAL4	NULL		bind	NULL	facilitated			nucleosomal templates	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_17_3520_s_420	11522821	45       Taylor,I.C.A., Workman,J.L., Schuetz,T.J. and Kingston,R.E. (1991) Facilitated binding of GAL4 and heat shock factor to nucleosomal templates: differential function of DNA binding domains.	bind
33343	2	8239	7	NULL	NULL	0	NULL	heat shock factor	NULL		bind	NULL	facilitated			nucleosomal templates	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_17_3520_s_420	11522821	45       Taylor,I.C.A., Workman,J.L., Schuetz,T.J. and Kingston,R.E. (1991) Facilitated binding of GAL4 and heat shock factor to nucleosomal templates: differential function of DNA binding domains.	bind
27330	1	8240	6	13	NULL	NULL	NULL	MSG1	GP		bind					p300/CBP coactivators	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_732_s_406	11160896	45       Yahata,T., de Caestecker,M.P., Lechleider,R.J., Andriole,S., Roberts,A.B., Isselbacher,K.J. and Shioda,T. (2000) The MSG1 non-DNA-binding transactivator binds to the p300/CBP coactivators, enhancing their functional link to the Smad transcription factors.	bind
27331	2	8240	6	13	NULL	NULL	NULL	MSG1	GP		is a type of					non-DNA-binding transactivator	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_732_s_406	11160896	45       Yahata,T., de Caestecker,M.P., Lechleider,R.J., Andriole,S., Roberts,A.B., Isselbacher,K.J. and Shioda,T. (2000) The MSG1 non-DNA-binding transactivator binds to the p300/CBP coactivators, enhancing their functional link to the Smad transcription factors.	bind
27332	3	8240	6	13	NULL	NULL	NULL	p300/CBP coactivators	GP		exhibit					Smad	GP	functional link to			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_732_s_406	11160896	45       Yahata,T., de Caestecker,M.P., Lechleider,R.J., Andriole,S., Roberts,A.B., Isselbacher,K.J. and Shioda,T. (2000) The MSG1 non-DNA-binding transactivator binds to the p300/CBP coactivators, enhancing their functional link to the Smad transcription factors.	bind
27333	4	8240	6	13	NULL	NULL	NULL	statement 1	Process		enhances					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_732_s_406	11160896	45       Yahata,T., de Caestecker,M.P., Lechleider,R.J., Andriole,S., Roberts,A.B., Isselbacher,K.J. and Shioda,T. (2000) The MSG1 non-DNA-binding transactivator binds to the p300/CBP coactivators, enhancing their functional link to the Smad transcription factors.	bind
46712	5	8240	6	13	NULL	NULL	NULL	Smad	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_732_s_406	11160896	45       Yahata,T., de Caestecker,M.P., Lechleider,R.J., Andriole,S., Roberts,A.B., Isselbacher,K.J. and Shioda,T. (2000) The MSG1 non-DNA-binding transactivator binds to the p300/CBP coactivators, enhancing their functional link to the Smad transcription factors.	bind
33344	1	8240	7	NULL	NULL	0	NULL	MSG1	NULL		binds	NULL				p300/CBP 	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_732_s_406	11160896	45       Yahata,T., de Caestecker,M.P., Lechleider,R.J., Andriole,S., Roberts,A.B., Isselbacher,K.J. and Shioda,T. (2000) The MSG1 non-DNA-binding transactivator binds to the p300/CBP coactivators, enhancing their functional link to the Smad transcription factors.	bind
33345	2	8240	7	NULL	NULL	0	NULL	MSG1	NULL		is a type of	NULL				non-DNA-binding transactivator	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_732_s_406	11160896	45       Yahata,T., de Caestecker,M.P., Lechleider,R.J., Andriole,S., Roberts,A.B., Isselbacher,K.J. and Shioda,T. (2000) The MSG1 non-DNA-binding transactivator binds to the p300/CBP coactivators, enhancing their functional link to the Smad transcription factors.	bind
33346	3	8240	7	NULL	NULL	0	NULL	p300/CBP 	NULL		is a type of	NULL				coactivator	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_732_s_406	11160896	45       Yahata,T., de Caestecker,M.P., Lechleider,R.J., Andriole,S., Roberts,A.B., Isselbacher,K.J. and Shioda,T. (2000) The MSG1 non-DNA-binding transactivator binds to the p300/CBP coactivators, enhancing their functional link to the Smad transcription factors.	bind
33347	4	8240	7	NULL	NULL	0	NULL	statement 1	NULL		enhance	NULL				Smad	NULL	functional link to			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_732_s_406	11160896	45       Yahata,T., de Caestecker,M.P., Lechleider,R.J., Andriole,S., Roberts,A.B., Isselbacher,K.J. and Shioda,T. (2000) The MSG1 non-DNA-binding transactivator binds to the p300/CBP coactivators, enhancing their functional link to the Smad transcription factors.	bind
33348	5	8240	7	NULL	NULL	0	NULL	Smad	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_732_s_406	11160896	45       Yahata,T., de Caestecker,M.P., Lechleider,R.J., Andriole,S., Roberts,A.B., Isselbacher,K.J. and Shioda,T. (2000) The MSG1 non-DNA-binding transactivator binds to the p300/CBP coactivators, enhancing their functional link to the Smad transcription factors.	bind
27334	1	8241	6	13	NULL	NULL	NULL	decorin	GP		bind					collagen	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_6_676_s_200	10747004	45  46  It also may be that the binding of decorin to collagen inhibits collagen degradation and stabilizes the collagen fibrillar network.	bind
27335	2	8241	6	13	NULL	NULL	NULL	statement 1	Process		inhibits		may			collagen 	GP	degradation of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_6_676_s_200	10747004	45  46  It also may be that the binding of decorin to collagen inhibits collagen degradation and stabilizes the collagen fibrillar network.	bind
27337	3	8241	6	13	NULL	NULL	NULL	statement 1	Process		stabilizes					collagen fibrillar network	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_6_676_s_200	10747004	45  46  It also may be that the binding of decorin to collagen inhibits collagen degradation and stabilizes the collagen fibrillar network.	bind
33351	1	8241	7	NULL	NULL	0	NULL	 decorin 	NULL		bind	NULL				collagen	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_86_6_676_s_200	10747004	45  46  It also may be that the binding of decorin to collagen inhibits collagen degradation and stabilizes the collagen fibrillar network.	bind
33352	2	8241	7	NULL	NULL	0	NULL	statement 1	NULL		inhibits	NULL				collagen	NULL	degradation of			NULL		0	NULL	NULL	NULL	gw60_circulationres_86_6_676_s_200	10747004	45  46  It also may be that the binding of decorin to collagen inhibits collagen degradation and stabilizes the collagen fibrillar network.	bind
33353	3	8241	7	NULL	NULL	0	NULL	statement 1	NULL		stabilizes	NULL				collagen fibrillar network	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_86_6_676_s_200	10747004	45  46  It also may be that the binding of decorin to collagen inhibits collagen degradation and stabilizes the collagen fibrillar network.	bind
27339	1	8242	6	13	NULL	NULL	NULL	heparin	Chemical		bind					thrombin	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1414_s_216	9261275	45  Although the amino acid sequences in heparin that bind to thrombin have not been identified, the oligosaccharide sequence in heparin that binds to antithrombin is quite different from that of LPL. 46  Thus, a specific set of monocyte surface HSPGs may bind to LPL and mediate monocyte adhesion.	bind
27340	2	8242	6	13	NULL	NULL	NULL	heparin	Chemical		bind			oligosaccharide sequence		antithrombin	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1414_s_216	9261275	45  Although the amino acid sequences in heparin that bind to thrombin have not been identified, the oligosaccharide sequence in heparin that binds to antithrombin is quite different from that of LPL. 46  Thus, a specific set of monocyte surface HSPGs may bind to LPL and mediate monocyte adhesion.	bind
27342	3	8242	6	13	NULL	NULL	NULL	HSPG	GP	monocyte surface	bind		may			LPL	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1414_s_216	9261275	45  Although the amino acid sequences in heparin that bind to thrombin have not been identified, the oligosaccharide sequence in heparin that binds to antithrombin is quite different from that of LPL. 46  Thus, a specific set of monocyte surface HSPGs may bind to LPL and mediate monocyte adhesion.	bind
27345	4	8242	6	13	NULL	NULL	NULL	statement 3	Process		mediate					monocyte	Cell	adhesion of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1414_s_216	9261275	45  Although the amino acid sequences in heparin that bind to thrombin have not been identified, the oligosaccharide sequence in heparin that binds to antithrombin is quite different from that of LPL. 46  Thus, a specific set of monocyte surface HSPGs may bind to LPL and mediate monocyte adhesion.	bind
46714	5	8242	6	13	NULL	NULL	NULL	heparin	Chemical		bind			oligosaccharide sequence		LPL	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1414_s_216	9261275	45  Although the amino acid sequences in heparin that bind to thrombin have not been identified, the oligosaccharide sequence in heparin that binds to antithrombin is quite different from that of LPL. 46  Thus, a specific set of monocyte surface HSPGs may bind to LPL and mediate monocyte adhesion.	bind
46715	6	8242	6	13	NULL	NULL	NULL	statement 2	Process	 	is different from					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1414_s_216	9261275	45  Although the amino acid sequences in heparin that bind to thrombin have not been identified, the oligosaccharide sequence in heparin that binds to antithrombin is quite different from that of LPL. 46  Thus, a specific set of monocyte surface HSPGs may bind to LPL and mediate monocyte adhesion.	bind
33356	1	8242	7	NULL	NULL	0	NULL	heparin	NULL		binds to	NULL				thrombin	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1414_s_216	9261275	45  Although the amino acid sequences in heparin that bind to thrombin have not been identified, the oligosaccharide sequence in heparin that binds to antithrombin is quite different from that of LPL. 46  Thus, a specific set of monocyte surface HSPGs may bind to LPL and mediate monocyte adhesion.	bind
33357	2	8242	7	10	NULL	0	NULL	heparin	NULL		binds to	NULL		oligosaccharide sequence		antithrombin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1414_s_216	9261275	45  Although the amino acid sequences in heparin that bind to thrombin have not been identified, the oligosaccharide sequence in heparin that binds to antithrombin is quite different from that of LPL. 46  Thus, a specific set of monocyte surface HSPGs may bind to LPL and mediate monocyte adhesion.	bind
33359	3	8242	7	10	NULL	0	NULL	heparin	NULL		binds to	NULL		oligosaccharide sequence		LPL	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1414_s_216	9261275	45  Although the amino acid sequences in heparin that bind to thrombin have not been identified, the oligosaccharide sequence in heparin that binds to antithrombin is quite different from that of LPL. 46  Thus, a specific set of monocyte surface HSPGs may bind to LPL and mediate monocyte adhesion.	bind
33366	4	8242	7	10	NULL	0	NULL	statement 2	NULL		is different from	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1414_s_216	9261275	45  Although the amino acid sequences in heparin that bind to thrombin have not been identified, the oligosaccharide sequence in heparin that binds to antithrombin is quite different from that of LPL. 46  Thus, a specific set of monocyte surface HSPGs may bind to LPL and mediate monocyte adhesion.	bind
33367	5	8242	7	NULL	NULL	0	NULL	HSPGs	NULL	monocyte surface	bind	NULL	may			LPL	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1414_s_216	9261275	45  Although the amino acid sequences in heparin that bind to thrombin have not been identified, the oligosaccharide sequence in heparin that binds to antithrombin is quite different from that of LPL. 46  Thus, a specific set of monocyte surface HSPGs may bind to LPL and mediate monocyte adhesion.	bind
33369	6	8242	7	10	NULL	0	NULL	statement 5	NULL		mediate	NULL				monocyte	NULL	adhesion of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1414_s_216	9261275	45  Although the amino acid sequences in heparin that bind to thrombin have not been identified, the oligosaccharide sequence in heparin that binds to antithrombin is quite different from that of LPL. 46  Thus, a specific set of monocyte surface HSPGs may bind to LPL and mediate monocyte adhesion.	bind
27347	1	8243	6	13	NULL	NULL	NULL	fibrinogen	GP		bind					GP IIb/IIa	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1532_s_297	8977459	45  Although we cannot totally exclude the possibility that a rapidly reversible fibrinogen binding to GP IIb/IIa was a factor in limiting aggregate size, our results with FITC-fibrinogen point more to a low degree of activation of GP IIb/IIa and to a level of fibrinogen binding insufficient to permit the formation of the macroaggregates.	bind
33372	1	8243	7	NULL	NULL	0	NULL	fibrinogen	NULL		bind	NULL	reversibly			GP IIb/IIa	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1532_s_297	8977459	45  Although we cannot totally exclude the possibility that a rapidly reversible fibrinogen binding to GP IIb/IIa was a factor in limiting aggregate size, our results with FITC-fibrinogen point more to a low degree of activation of GP IIb/IIa and to a level of fibrinogen binding insufficient to permit the formation of the macroaggregates.	bind
33374	2	8243	7	NULL	NULL	0	NULL	statement 1	NULL		limits	NULL				aggregate size	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1532_s_297	8977459	45  Although we cannot totally exclude the possibility that a rapidly reversible fibrinogen binding to GP IIb/IIa was a factor in limiting aggregate size, our results with FITC-fibrinogen point more to a low degree of activation of GP IIb/IIa and to a level of fibrinogen binding insufficient to permit the formation of the macroaggregates.	bind
33375	3	8243	7	NULL	NULL	0	NULL	statement 1	NULL		insufficient to permit	NULL				macroaggregates	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1532_s_297	8977459	45  Although we cannot totally exclude the possibility that a rapidly reversible fibrinogen binding to GP IIb/IIa was a factor in limiting aggregate size, our results with FITC-fibrinogen point more to a low degree of activation of GP IIb/IIa and to a level of fibrinogen binding insufficient to permit the formation of the macroaggregates.	bind
27352	1	8244	6	13	NULL	NULL	NULL	fibrinogen	GP		bind					GP IIb/IIIa	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_4_437_s_123	10421606	45  LIBS epitope expression seems to be a normal function of GP IIb/IIa, as evidenced by observations showing that fibrinogen binding to GP IIb/IIIa also induces this effect.	bind
27353	2	8244	6	13	NULL	NULL	NULL	GP IIb/IIa	GP		expresses					LIBS epitope	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_4_437_s_123	10421606	45  LIBS epitope expression seems to be a normal function of GP IIb/IIa, as evidenced by observations showing that fibrinogen binding to GP IIb/IIIa also induces this effect.	bind
27354	3	8244	6	13	NULL	NULL	NULL	statement 1	Process		induces					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_4_437_s_123	10421606	45  LIBS epitope expression seems to be a normal function of GP IIb/IIa, as evidenced by observations showing that fibrinogen binding to GP IIb/IIIa also induces this effect.	bind
33378	1	8244	7	NULL	NULL	0	NULL	fibrinogen	NULL		bind	NULL				GP IIb/IIIa	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_100_4_437_s_123	10421606	45  LIBS epitope expression seems to be a normal function of GP IIb/IIa, as evidenced by observations showing that fibrinogen binding to GP IIb/IIIa also induces this effect.	bind
46717	2	8244	7	10	NULL	0	NULL	GP IIb/IIa	NULL		express	NULL				LIBS epitope	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_100_4_437_s_123	10421606	45  LIBS epitope expression seems to be a normal function of GP IIb/IIa, as evidenced by observations showing that fibrinogen binding to GP IIb/IIIa also induces this effect.	bind
46718	3	8244	7	10	NULL	0	NULL	statement 1	NULL		induce	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_100_4_437_s_123	10421606	45  LIBS epitope expression seems to be a normal function of GP IIb/IIa, as evidenced by observations showing that fibrinogen binding to GP IIb/IIIa also induces this effect.	bind
27355	1	8245	6	13	NULL	NULL	NULL	PEA-3	GP		bind					ets	GP			consensus binding site	NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_6_1777_s_171	11106549	45  PEA-3, another transcription factor that binds to the ets consensus binding site, has been shown by Trimble et al to be overexpressed in the mammary carcinomas that result from expression of the MMTV-polyoma middle T transgene, making it an attractive candidate for involvement in the induction of MMP-9 promoter activity during tumor progression.	bind
27357	2	8245	6	13	NULL	NULL	NULL	PEA-3	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_6_1777_s_171	11106549	45  PEA-3, another transcription factor that binds to the ets consensus binding site, has been shown by Trimble et al to be overexpressed in the mammary carcinomas that result from expression of the MMTV-polyoma middle T transgene, making it an attractive candidate for involvement in the induction of MMP-9 promoter activity during tumor progression.	bind
27362	3	8245	6	13	NULL	NULL	NULL	PEA-3	GP		is overexpressed in					mammary carcinomas	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_6_1777_s_171	11106549	45  PEA-3, another transcription factor that binds to the ets consensus binding site, has been shown by Trimble et al to be overexpressed in the mammary carcinomas that result from expression of the MMTV-polyoma middle T transgene, making it an attractive candidate for involvement in the induction of MMP-9 promoter activity during tumor progression.	bind
27366	4	8245	6	13	NULL	NULL	NULL	PEA-3	GP		is involved in					MMP-9	GP	induction of;; activity of		promoter	NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_6_1777_s_171	11106549	45  PEA-3, another transcription factor that binds to the ets consensus binding site, has been shown by Trimble et al to be overexpressed in the mammary carcinomas that result from expression of the MMTV-polyoma middle T transgene, making it an attractive candidate for involvement in the induction of MMP-9 promoter activity during tumor progression.	bind
27368	5	8245	6	13	NULL	NULL	NULL	statement 4	Process		occurs during					tumor progression	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_6_1777_s_171	11106549	45  PEA-3, another transcription factor that binds to the ets consensus binding site, has been shown by Trimble et al to be overexpressed in the mammary carcinomas that result from expression of the MMTV-polyoma middle T transgene, making it an attractive candidate for involvement in the induction of MMP-9 promoter activity during tumor progression.	bind
55954	6	8245	6	13	NULL	NULL	NULL	statement 3	Process		results from					MMTV-polyoma middle T transgene	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_6_1777_s_171	11106549	45  PEA-3, another transcription factor that binds to the ets consensus binding site, has been shown by Trimble et al to be overexpressed in the mammary carcinomas that result from expression of the MMTV-polyoma middle T transgene, making it an attractive candidate for involvement in the induction of MMP-9 promoter activity during tumor progression.	bind
33381	1	8245	7	10	NULL	0	NULL	 PEA-3			binds to					ets				consensus binding site	NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_6_1777_s_171	11106549	45  PEA-3, another transcription factor that binds to the ets consensus binding site, has been shown by Trimble et al to be overexpressed in the mammary carcinomas that result from expression of the MMTV-polyoma middle T transgene, making it an attractive candidate for involvement in the induction of MMP-9 promoter activity during tumor progression.	bind
33382	2	8245	7	NULL	NULL	0	NULL	PEA-3	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_6_1777_s_171	11106549	45  PEA-3, another transcription factor that binds to the ets consensus binding site, has been shown by Trimble et al to be overexpressed in the mammary carcinomas that result from expression of the MMTV-polyoma middle T transgene, making it an attractive candidate for involvement in the induction of MMP-9 promoter activity during tumor progression.	bind
33383	3	8245	7	10	NULL	0	NULL	statement  6			result from					MMTV-polyoma middle T transgene		expression of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_6_1777_s_171	11106549	45  PEA-3, another transcription factor that binds to the ets consensus binding site, has been shown by Trimble et al to be overexpressed in the mammary carcinomas that result from expression of the MMTV-polyoma middle T transgene, making it an attractive candidate for involvement in the induction of MMP-9 promoter activity during tumor progression.	bind
33463	4	8245	7	10	NULL	0	NULL	 PEA-3			is involved in					MMP-9 		induction of;;activity of		promoter	NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_6_1777_s_171	11106549	45  PEA-3, another transcription factor that binds to the ets consensus binding site, has been shown by Trimble et al to be overexpressed in the mammary carcinomas that result from expression of the MMTV-polyoma middle T transgene, making it an attractive candidate for involvement in the induction of MMP-9 promoter activity during tumor progression.	bind
33464	5	8245	7	NULL	NULL	0	NULL	statement 4	NULL		occurs during	NULL				tumor progression	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_6_1777_s_171	11106549	45  PEA-3, another transcription factor that binds to the ets consensus binding site, has been shown by Trimble et al to be overexpressed in the mammary carcinomas that result from expression of the MMTV-polyoma middle T transgene, making it an attractive candidate for involvement in the induction of MMP-9 promoter activity during tumor progression.	bind
55953	6	8245	7	10	NULL	0	NULL	PEA-3			is overexpressed in					mammary carcinomas					NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_6_1777_s_171	11106549	45  PEA-3, another transcription factor that binds to the ets consensus binding site, has been shown by Trimble et al to be overexpressed in the mammary carcinomas that result from expression of the MMTV-polyoma middle T transgene, making it an attractive candidate for involvement in the induction of MMP-9 promoter activity during tumor progression.	bind
27370	1	8246	6	13	NULL	NULL	NULL	LDL	GP		bind					PG	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_1053_s_143	11397719	45  Surprisingly, as shown in this study, after prolonged incubation (36 hours), mere binding of LDL to PGs can induce aggregation of a fraction of the LDL particles.	bind
27371	2	8246	6	13	NULL	NULL	NULL	statement 1	Process		induce					LDL particles	GP	aggregation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_1053_s_143	11397719	45  Surprisingly, as shown in this study, after prolonged incubation (36 hours), mere binding of LDL to PGs can induce aggregation of a fraction of the LDL particles.	bind
33465	1	8246	7	NULL	NULL	0	NULL	LDL	NULL		bind	NULL				PGs	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_1053_s_143	11397719	45  Surprisingly, as shown in this study, after prolonged incubation (36 hours), mere binding of LDL to PGs can induce aggregation of a fraction of the LDL particles.	bind
33466	2	8246	7	NULL	NULL	0	NULL	statement 1	NULL		induce	NULL				LDL particles	NULL	aggregation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_6_1053_s_143	11397719	45  Surprisingly, as shown in this study, after prolonged incubation (36 hours), mere binding of LDL to PGs can induce aggregation of a fraction of the LDL particles.	bind
27372	1	8247	6	13	NULL	NULL	NULL	Mox1 protein	GP		bind		directly	 		Pax1 protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_6_2181_s_241	12057921	45  The Mox1 and Mox2 proteins bind directly to Pax1 and Pax3 proteins, respectively.	bind
27374	2	8247	6	13	NULL	NULL	NULL	Mox2 protein	GP		bind		directly			Pax3 protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_6_2181_s_241	12057921	45  The Mox1 and Mox2 proteins bind directly to Pax1 and Pax3 proteins, respectively.	bind
33467	1	8247	7	NULL	NULL	0	NULL	Mox1 protein	NULL		bind	NULL	directly			Pax1 protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_6_2181_s_241	12057921	45  The Mox1 and Mox2 proteins bind directly to Pax1 and Pax3 proteins, respectively.	bind
33468	2	8247	7	NULL	NULL	0	NULL	Mox2 protein	NULL		bind	NULL	directly			Pax3 protein	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_6_2181_s_241	12057921	45  The Mox1 and Mox2 proteins bind directly to Pax1 and Pax3 proteins, respectively.	bind
27378	1	8248	6	13	NULL	NULL	NULL	endothelial cells	Cell		produce					1MCP-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_9_2488_s_50	7729036	45 47  Moreover, mildly oxidized LDL induced endothelial cells to produce the potent monocyte activators monocyte chemoattractant protein (1MCP-1), 48  monocyte colony stimulating factor (M-CSF), 49  and GRO. 50  While M-CSF and MCP-1 appear to be soluble molecules, GRO was found bound to heparin-like molecules on the endothelial cell surface.	bind
27381	2	8248	6	13	NULL	NULL	NULL	endothelial cells	Cell		produce					M-CSF	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_9_2488_s_50	7729036	45 47  Moreover, mildly oxidized LDL induced endothelial cells to produce the potent monocyte activators monocyte chemoattractant protein (1MCP-1), 48  monocyte colony stimulating factor (M-CSF), 49  and GRO. 50  While M-CSF and MCP-1 appear to be soluble molecules, GRO was found bound to heparin-like molecules on the endothelial cell surface.	bind
27382	3	8248	6	13	NULL	NULL	NULL	endothelial cells	Cell		produce					GRO	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_9_2488_s_50	7729036	45 47  Moreover, mildly oxidized LDL induced endothelial cells to produce the potent monocyte activators monocyte chemoattractant protein (1MCP-1), 48  monocyte colony stimulating factor (M-CSF), 49  and GRO. 50  While M-CSF and MCP-1 appear to be soluble molecules, GRO was found bound to heparin-like molecules on the endothelial cell surface.	bind
27383	4	8248	6	13	NULL	NULL	NULL	LDL	GP	mildly oxidized	induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_9_2488_s_50	7729036	45 47  Moreover, mildly oxidized LDL induced endothelial cells to produce the potent monocyte activators monocyte chemoattractant protein (1MCP-1), 48  monocyte colony stimulating factor (M-CSF), 49  and GRO. 50  While M-CSF and MCP-1 appear to be soluble molecules, GRO was found bound to heparin-like molecules on the endothelial cell surface.	bind
27384	5	8248	6	13	NULL	NULL	NULL	LDL	GP	mildly oxidized	induce					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_9_2488_s_50	7729036	45 47  Moreover, mildly oxidized LDL induced endothelial cells to produce the potent monocyte activators monocyte chemoattractant protein (1MCP-1), 48  monocyte colony stimulating factor (M-CSF), 49  and GRO. 50  While M-CSF and MCP-1 appear to be soluble molecules, GRO was found bound to heparin-like molecules on the endothelial cell surface.	bind
27385	6	8248	6	13	NULL	NULL	NULL	LDL	GP	mildly oxidized	induce					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_9_2488_s_50	7729036	45 47  Moreover, mildly oxidized LDL induced endothelial cells to produce the potent monocyte activators monocyte chemoattractant protein (1MCP-1), 48  monocyte colony stimulating factor (M-CSF), 49  and GRO. 50  While M-CSF and MCP-1 appear to be soluble molecules, GRO was found bound to heparin-like molecules on the endothelial cell surface.	bind
27387	7	8248	6	13	NULL	NULL	NULL	GRO	GP		bind					heparin-like molecules	GP				NULL	endothelial cell surface	NULL	NULL	NULL	NULL	gw60_circulation_91_9_2488_s_50	7729036	45 47  Moreover, mildly oxidized LDL induced endothelial cells to produce the potent monocyte activators monocyte chemoattractant protein (1MCP-1), 48  monocyte colony stimulating factor (M-CSF), 49  and GRO. 50  While M-CSF and MCP-1 appear to be soluble molecules, GRO was found bound to heparin-like molecules on the endothelial cell surface.	bind
27390	8	8248	6	13	NULL	NULL	NULL	1MCP-1	GP		is					monocyte chemoattractant protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_9_2488_s_50	7729036	45 47  Moreover, mildly oxidized LDL induced endothelial cells to produce the potent monocyte activators monocyte chemoattractant protein (1MCP-1), 48  monocyte colony stimulating factor (M-CSF), 49  and GRO. 50  While M-CSF and MCP-1 appear to be soluble molecules, GRO was found bound to heparin-like molecules on the endothelial cell surface.	bind
27392	9	8248	6	13	NULL	NULL	NULL	M-CSF	GP		is					monocyte colony stimulating factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_9_2488_s_50	7729036	45 47  Moreover, mildly oxidized LDL induced endothelial cells to produce the potent monocyte activators monocyte chemoattractant protein (1MCP-1), 48  monocyte colony stimulating factor (M-CSF), 49  and GRO. 50  While M-CSF and MCP-1 appear to be soluble molecules, GRO was found bound to heparin-like molecules on the endothelial cell surface.	bind
27393	10	8248	6	13	NULL	NULL	NULL	M-CSF	GP		is a type of					soluble molecule	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_9_2488_s_50	7729036	45 47  Moreover, mildly oxidized LDL induced endothelial cells to produce the potent monocyte activators monocyte chemoattractant protein (1MCP-1), 48  monocyte colony stimulating factor (M-CSF), 49  and GRO. 50  While M-CSF and MCP-1 appear to be soluble molecules, GRO was found bound to heparin-like molecules on the endothelial cell surface.	bind
27395	11	8248	6	13	NULL	NULL	NULL	1MCP-1	GP		is a type of					soluble molecule	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_9_2488_s_50	7729036	45 47  Moreover, mildly oxidized LDL induced endothelial cells to produce the potent monocyte activators monocyte chemoattractant protein (1MCP-1), 48  monocyte colony stimulating factor (M-CSF), 49  and GRO. 50  While M-CSF and MCP-1 appear to be soluble molecules, GRO was found bound to heparin-like molecules on the endothelial cell surface.	bind
46719	12	8248	6	13	NULL	NULL	NULL	1MCP-1	GP		is a type of					monocyte activator	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_9_2488_s_50	7729036	45 47  Moreover, mildly oxidized LDL induced endothelial cells to produce the potent monocyte activators monocyte chemoattractant protein (1MCP-1), 48  monocyte colony stimulating factor (M-CSF), 49  and GRO. 50  While M-CSF and MCP-1 appear to be soluble molecules, GRO was found bound to heparin-like molecules on the endothelial cell surface.	bind
46720	13	8248	6	13	NULL	NULL	NULL	M-CSF	GP		is a type of					monocyte activator	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_9_2488_s_50	7729036	45 47  Moreover, mildly oxidized LDL induced endothelial cells to produce the potent monocyte activators monocyte chemoattractant protein (1MCP-1), 48  monocyte colony stimulating factor (M-CSF), 49  and GRO. 50  While M-CSF and MCP-1 appear to be soluble molecules, GRO was found bound to heparin-like molecules on the endothelial cell surface.	bind
33469	1	8248	7	10	NULL	0	NULL	LDL		mildly oxidized	induce					endothelial cells					NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_9_2488_s_50	7729036	45 47  Moreover, mildly oxidized LDL induced endothelial cells to produce the potent monocyte activators monocyte chemoattractant protein (1MCP-1), 48  monocyte colony stimulating factor (M-CSF), 49  and GRO. 50  While M-CSF and MCP-1 appear to be soluble molecules, GRO was found bound to heparin-like molecules on the endothelial cell surface.	bind
33470	2	8248	7	NULL	NULL	0	NULL	statement 1	NULL		produce	NULL				1MCP-1	NULL	potent			NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_9_2488_s_50	7729036	45 47  Moreover, mildly oxidized LDL induced endothelial cells to produce the potent monocyte activators monocyte chemoattractant protein (1MCP-1), 48  monocyte colony stimulating factor (M-CSF), 49  and GRO. 50  While M-CSF and MCP-1 appear to be soluble molecules, GRO was found bound to heparin-like molecules on the endothelial cell surface.	bind
33471	3	8248	7	NULL	NULL	0	NULL	statement 1	NULL		produce	NULL				M-CSF	NULL	potent			NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_9_2488_s_50	7729036	45 47  Moreover, mildly oxidized LDL induced endothelial cells to produce the potent monocyte activators monocyte chemoattractant protein (1MCP-1), 48  monocyte colony stimulating factor (M-CSF), 49  and GRO. 50  While M-CSF and MCP-1 appear to be soluble molecules, GRO was found bound to heparin-like molecules on the endothelial cell surface.	bind
33472	4	8248	7	NULL	NULL	0	NULL	statement 1	NULL		produce	NULL				GRO	NULL	potent			NULL		0	NULL	NULL	NULL	gw60_circulation_91_9_2488_s_50	7729036	45 47  Moreover, mildly oxidized LDL induced endothelial cells to produce the potent monocyte activators monocyte chemoattractant protein (1MCP-1), 48  monocyte colony stimulating factor (M-CSF), 49  and GRO. 50  While M-CSF and MCP-1 appear to be soluble molecules, GRO was found bound to heparin-like molecules on the endothelial cell surface.	bind
33473	5	8248	7	NULL	NULL	0	NULL	1MCP-1	NULL		is a type of	NULL				monocyte activators	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_91_9_2488_s_50	7729036	45 47  Moreover, mildly oxidized LDL induced endothelial cells to produce the potent monocyte activators monocyte chemoattractant protein (1MCP-1), 48  monocyte colony stimulating factor (M-CSF), 49  and GRO. 50  While M-CSF and MCP-1 appear to be soluble molecules, GRO was found bound to heparin-like molecules on the endothelial cell surface.	bind
33474	6	8248	7	NULL	NULL	0	NULL	M-CSF	NULL		is a type of	NULL				 monocyte activators	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_91_9_2488_s_50	7729036	45 47  Moreover, mildly oxidized LDL induced endothelial cells to produce the potent monocyte activators monocyte chemoattractant protein (1MCP-1), 48  monocyte colony stimulating factor (M-CSF), 49  and GRO. 50  While M-CSF and MCP-1 appear to be soluble molecules, GRO was found bound to heparin-like molecules on the endothelial cell surface.	bind
33475	7	8248	7	NULL	NULL	0	NULL	1MCP-1	NULL		is	NULL				monocyte chemoattractant protein	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_91_9_2488_s_50	7729036	45 47  Moreover, mildly oxidized LDL induced endothelial cells to produce the potent monocyte activators monocyte chemoattractant protein (1MCP-1), 48  monocyte colony stimulating factor (M-CSF), 49  and GRO. 50  While M-CSF and MCP-1 appear to be soluble molecules, GRO was found bound to heparin-like molecules on the endothelial cell surface.	bind
33476	8	8248	7	NULL	NULL	0	NULL	M-CSF	NULL		is	NULL				monocyte colony stimulating factor 	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_91_9_2488_s_50	7729036	45 47  Moreover, mildly oxidized LDL induced endothelial cells to produce the potent monocyte activators monocyte chemoattractant protein (1MCP-1), 48  monocyte colony stimulating factor (M-CSF), 49  and GRO. 50  While M-CSF and MCP-1 appear to be soluble molecules, GRO was found bound to heparin-like molecules on the endothelial cell surface.	bind
33477	9	8248	7	NULL	NULL	0	NULL	GRO	NULL		bind	NULL				heparin-like molecules	NULL				NULL	endothelial cell surface	0	NULL	NULL	NULL	gw60_circulation_91_9_2488_s_50	7729036	45 47  Moreover, mildly oxidized LDL induced endothelial cells to produce the potent monocyte activators monocyte chemoattractant protein (1MCP-1), 48  monocyte colony stimulating factor (M-CSF), 49  and GRO. 50  While M-CSF and MCP-1 appear to be soluble molecules, GRO was found bound to heparin-like molecules on the endothelial cell surface.	bind
33478	10	8248	7	NULL	NULL	0	NULL	M-CSF	NULL		is a type of	NULL				soluble molecule	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_91_9_2488_s_50	7729036	45 47  Moreover, mildly oxidized LDL induced endothelial cells to produce the potent monocyte activators monocyte chemoattractant protein (1MCP-1), 48  monocyte colony stimulating factor (M-CSF), 49  and GRO. 50  While M-CSF and MCP-1 appear to be soluble molecules, GRO was found bound to heparin-like molecules on the endothelial cell surface.	bind
33479	11	8248	7	NULL	NULL	0	NULL	MCP-1	NULL		is a type of	NULL				soluble molecule	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_91_9_2488_s_50	7729036	45 47  Moreover, mildly oxidized LDL induced endothelial cells to produce the potent monocyte activators monocyte chemoattractant protein (1MCP-1), 48  monocyte colony stimulating factor (M-CSF), 49  and GRO. 50  While M-CSF and MCP-1 appear to be soluble molecules, GRO was found bound to heparin-like molecules on the endothelial cell surface.	bind
27399	1	8249	6	13	NULL	NULL	NULL	Keap1	GP		bind					actin cytoskeleton	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_10_967_s_145	16284189	45 Curiously, Keap1 is a cysteine-rich protein that can bind to the actin cytoskeleton in addition to binding to Nrf2.	bind
27403	2	8249	6	13	NULL	NULL	NULL	Keap1	GP		is a type of					cysteine-rich protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_10_967_s_145	16284189	45 Curiously, Keap1 is a cysteine-rich protein that can bind to the actin cytoskeleton in addition to binding to Nrf2.	bind
27404	3	8249	6	13	NULL	NULL	NULL	Keap1	GP		bind					Nrf2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_10_967_s_145	16284189	45 Curiously, Keap1 is a cysteine-rich protein that can bind to the actin cytoskeleton in addition to binding to Nrf2.	bind
33480	1	8249	7	NULL	NULL	0	NULL	Keap1	NULL		bind	NULL				actin cytoskeleton	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_10_967_s_145	16284189	45 Curiously, Keap1 is a cysteine-rich protein that can bind to the actin cytoskeleton in addition to binding to Nrf2.	bind
33481	2	8249	7	NULL	NULL	0	NULL	 Keap1	NULL		bind	NULL				Nrf2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_10_967_s_145	16284189	45 Curiously, Keap1 is a cysteine-rich protein that can bind to the actin cytoskeleton in addition to binding to Nrf2.	bind
33482	3	8249	7	NULL	NULL	0	NULL	Keap1	NULL		is a type of	NULL				cysteine-rich protein	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_10_967_s_145	16284189	45 Curiously, Keap1 is a cysteine-rich protein that can bind to the actin cytoskeleton in addition to binding to Nrf2.	bind
27406	1	8250	6	13	NULL	NULL	NULL	HIF-1	GP		bind					VEGF	GP			hypoxia-response element of promoter	NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_16_2477_s_205	16230500	45 Hypoxia upregulates  VEGF gene transcription by activating the hypoxia-inducible transcription factors HIF-1 and HIF-2, which bind the hypoxia-response element in the  VEGF promotor.	bind
27408	2	8250	6	13	NULL	NULL	NULL	HIF-2	GP		bind					VEGF	GP			hypoxia-response element of promoter	NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_16_2477_s_205	16230500	45 Hypoxia upregulates  VEGF gene transcription by activating the hypoxia-inducible transcription factors HIF-1 and HIF-2, which bind the hypoxia-response element in the  VEGF promotor.	bind
27450	3	8250	6	13	NULL	NULL	NULL	hypoxia	MedicalFinding		upregulates					VEGF gene	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_16_2477_s_205	16230500	45 Hypoxia upregulates  VEGF gene transcription by activating the hypoxia-inducible transcription factors HIF-1 and HIF-2, which bind the hypoxia-response element in the  VEGF promotor.	bind
46722	4	8250	6	13	NULL	NULL	NULL	statement 1	Process		occurs by					HIF-1	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_16_2477_s_205	16230500	45 Hypoxia upregulates  VEGF gene transcription by activating the hypoxia-inducible transcription factors HIF-1 and HIF-2, which bind the hypoxia-response element in the  VEGF promotor.	bind
46723	5	8250	6	13	NULL	NULL	NULL	statement 1	Process		occurs by					HIF-2	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_16_2477_s_205	16230500	45 Hypoxia upregulates  VEGF gene transcription by activating the hypoxia-inducible transcription factors HIF-1 and HIF-2, which bind the hypoxia-response element in the  VEGF promotor.	bind
33483	1	8250	7	10	NULL	0	NULL	Hypoxia	NULL		upregulates	NULL				VEGF gene	NULL	transcription of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_16_2477_s_205	16230500	45 Hypoxia upregulates  VEGF gene transcription by activating the hypoxia-inducible transcription factors HIF-1 and HIF-2, which bind the hypoxia-response element in the  VEGF promotor.	bind
33484	2	8250	7	NULL	NULL	0	NULL	HIF-1	NULL		bind	NULL				VEGF	NULL			hypoxia-response element in the promoter	NULL		0	NULL	NULL	NULL	gw70_circulation_112_16_2477_s_205	16230500	45 Hypoxia upregulates  VEGF gene transcription by activating the hypoxia-inducible transcription factors HIF-1 and HIF-2, which bind the hypoxia-response element in the  VEGF promotor.	bind
33485	3	8250	7	NULL	NULL	0	NULL	HIF-2	NULL		bind	NULL				VEGF	NULL			hypoxia-response element in the promoter	NULL		0	NULL	NULL	NULL	gw70_circulation_112_16_2477_s_205	16230500	45 Hypoxia upregulates  VEGF gene transcription by activating the hypoxia-inducible transcription factors HIF-1 and HIF-2, which bind the hypoxia-response element in the  VEGF promotor.	bind
33486	4	8250	7	10	NULL	0	NULL	statement 1	NULL		occurs by	NULL				HIF-1	NULL	activation of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_16_2477_s_205	16230500	45 Hypoxia upregulates  VEGF gene transcription by activating the hypoxia-inducible transcription factors HIF-1 and HIF-2, which bind the hypoxia-response element in the  VEGF promotor.	bind
33487	5	8250	7	10	NULL	0	NULL	statement 1	NULL		occurs by	NULL				HIF-2	NULL	activation of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_16_2477_s_205	16230500	45 Hypoxia upregulates  VEGF gene transcription by activating the hypoxia-inducible transcription factors HIF-1 and HIF-2, which bind the hypoxia-response element in the  VEGF promotor.	bind
27459	1	8251	6	13	NULL	NULL	NULL	FAK	GP		bind			amino terminus		RIP	GP		death domain		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_5_606_s_82	16543511	45,46,55   The FAK amino terminus binds to the death domain of RIP, and prevents RIP interaction with the Fas-containing death complex, 56 and the FAK N-terminus also binds to the transactivation domain of p53 to block activation of the Bax promoter.	bind
27462	2	8251	6	13	NULL	NULL	NULL	FAK	GP		bind			N terminus		p53	GP		transactivation domain		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_5_606_s_82	16543511	45,46,55   The FAK amino terminus binds to the death domain of RIP, and prevents RIP interaction with the Fas-containing death complex, 56 and the FAK N-terminus also binds to the transactivation domain of p53 to block activation of the Bax promoter.	bind
27465	3	8251	6	13	NULL	NULL	NULL	statement 2	Process		block					Bax promoter	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_5_606_s_82	16543511	45,46,55   The FAK amino terminus binds to the death domain of RIP, and prevents RIP interaction with the Fas-containing death complex, 56 and the FAK N-terminus also binds to the transactivation domain of p53 to block activation of the Bax promoter.	bind
27466	4	8251	6	13	NULL	NULL	NULL	RIP	GP		interacts with					Fas-containing death complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_5_606_s_82	16543511	45,46,55   The FAK amino terminus binds to the death domain of RIP, and prevents RIP interaction with the Fas-containing death complex, 56 and the FAK N-terminus also binds to the transactivation domain of p53 to block activation of the Bax promoter.	bind
27467	5	8251	6	13	NULL	NULL	NULL	statement 1	Process		prevents					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_5_606_s_82	16543511	45,46,55   The FAK amino terminus binds to the death domain of RIP, and prevents RIP interaction with the Fas-containing death complex, 56 and the FAK N-terminus also binds to the transactivation domain of p53 to block activation of the Bax promoter.	bind
33488	1	8251	7	NULL	NULL	0	NULL	FAK	NULL		binds to	NULL		amino terminus		RIP	NULL		death domain		NULL		0	NULL	NULL	NULL	gw70_circulationres_98_5_606_s_82	16543511	45,46,55   The FAK amino terminus binds to the death domain of RIP, and prevents RIP interaction with the Fas-containing death complex, 56 and the FAK N-terminus also binds to the transactivation domain of p53 to block activation of the Bax promoter.	bind
33489	2	8251	7	NULL	NULL	0	NULL	RIP	NULL		interacts with	NULL				Fas-containing death complex	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_5_606_s_82	16543511	45,46,55   The FAK amino terminus binds to the death domain of RIP, and prevents RIP interaction with the Fas-containing death complex, 56 and the FAK N-terminus also binds to the transactivation domain of p53 to block activation of the Bax promoter.	bind
33490	3	8251	7	NULL	NULL	0	NULL	statement 1	NULL		prevents	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_5_606_s_82	16543511	45,46,55   The FAK amino terminus binds to the death domain of RIP, and prevents RIP interaction with the Fas-containing death complex, 56 and the FAK N-terminus also binds to the transactivation domain of p53 to block activation of the Bax promoter.	bind
33491	4	8251	7	NULL	NULL	0	NULL	FAK	NULL		binds to	NULL		N-terminus		p53	NULL		transactivation domain		NULL		0	NULL	NULL	NULL	gw70_circulationres_98_5_606_s_82	16543511	45,46,55   The FAK amino terminus binds to the death domain of RIP, and prevents RIP interaction with the Fas-containing death complex, 56 and the FAK N-terminus also binds to the transactivation domain of p53 to block activation of the Bax promoter.	bind
33492	5	8251	7	NULL	NULL	0	NULL	statement 4	NULL		block	NULL				Bax	NULL	activation of		promoter	NULL		0	NULL	NULL	NULL	gw70_circulationres_98_5_606_s_82	16543511	45,46,55   The FAK amino terminus binds to the death domain of RIP, and prevents RIP interaction with the Fas-containing death complex, 56 and the FAK N-terminus also binds to the transactivation domain of p53 to block activation of the Bax promoter.	bind
47079	1	8252	6	13	NULL	NULL	NULL	Ca2+	Chemical		bind					GST-PLDbeta proteins	GP	engineered			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_46_47833_s_70	15356005	45Ca2+ Binding Assay -- 45Ca2+ binding of the engineered GST-PLDbeta proteins and GST was evaluated using a described method with some modifications ( ,  ).	bind
33493	1	8252	7	10	NULL	0	NULL	Ca2+			bind					GST-PLDbeta proteins		engineered			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_46_47833_s_70	15356005	45Ca2+ Binding Assay -- 45Ca2+ binding of the engineered GST-PLDbeta proteins and GST was evaluated using a described method with some modifications ( ,  ).	bind
27468	1	8253	6	13	NULL	NULL	NULL	ORC	GP	drosophila	bind		specifically			ACE3	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_809_s_393	11160905	46       Austin,R.J., Orr-Weaver,T.L. and Bell,S.P. (1999) Drosophila ORC specifically binds to ACE3, an origin of DNA replication control element.	bind
27469	2	8253	6	13	NULL	NULL	NULL	ACE3	GP		is a type of					origin of DNA replication control element	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_809_s_393	11160905	46       Austin,R.J., Orr-Weaver,T.L. and Bell,S.P. (1999) Drosophila ORC specifically binds to ACE3, an origin of DNA replication control element.	bind
33494	1	8253	7	NULL	NULL	0	NULL	ORC	NULL	Drosophila	binds	NULL	specifically			ACE3	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_809_s_393	11160905	46       Austin,R.J., Orr-Weaver,T.L. and Bell,S.P. (1999) Drosophila ORC specifically binds to ACE3, an origin of DNA replication control element.	bind
33495	2	8253	7	10	NULL	0	NULL	ACE3	NULL		is a type of	NULL				origin of DNA replication control element	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_809_s_393	11160905	46       Austin,R.J., Orr-Weaver,T.L. and Bell,S.P. (1999) Drosophila ORC specifically binds to ACE3, an origin of DNA replication control element.	bind
27470	1	8254	6	13	NULL	NULL	NULL	high mobility group 1 protein	GP		bind					DNA	NucleicAcid	cisplatin-modified			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_5_1200_s_407	11222770	46       Imamura,T., Izumi,H., Nagatani,G., Ise,T., Nomoto,M., Iwamoto,Y. and Kohno,K. (2001) Interaction with p53 enhances binding of cisplatin-modified DNA by high mobility group 1 protein.	bind
27471	2	8254	6	13	NULL	NULL	NULL	DNA	NucleicAcid	cisplatin modified	interacts with					p53	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_5_1200_s_407	11222770	46       Imamura,T., Izumi,H., Nagatani,G., Ise,T., Nomoto,M., Iwamoto,Y. and Kohno,K. (2001) Interaction with p53 enhances binding of cisplatin-modified DNA by high mobility group 1 protein.	bind
27472	3	8254	6	13	NULL	NULL	NULL	statement 2	Process		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_5_1200_s_407	11222770	46       Imamura,T., Izumi,H., Nagatani,G., Ise,T., Nomoto,M., Iwamoto,Y. and Kohno,K. (2001) Interaction with p53 enhances binding of cisplatin-modified DNA by high mobility group 1 protein.	bind
33496	1	8254	7	10	NULL	0	NULL	high mobility group 1 protein	NULL		bind	NULL				DNA	NULL	cisplatin-modified			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_5_1200_s_407	11222770	46       Imamura,T., Izumi,H., Nagatani,G., Ise,T., Nomoto,M., Iwamoto,Y. and Kohno,K. (2001) Interaction with p53 enhances binding of cisplatin-modified DNA by high mobility group 1 protein.	bind
33497	2	8254	7	NULL	NULL	0	NULL	p53	NULL		enhances	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_5_1200_s_407	11222770	46       Imamura,T., Izumi,H., Nagatani,G., Ise,T., Nomoto,M., Iwamoto,Y. and Kohno,K. (2001) Interaction with p53 enhances binding of cisplatin-modified DNA by high mobility group 1 protein.	bind
27473	1	8257	6	13	NULL	NULL	NULL	VEGF-D	GP	human	bind					VEGFR-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_4_1405_s_373	11943725	46  Human VEGF-D binds and activates VEGFR-2 and VEGFR-3, suggesting roles in angiogenesis and lymphangiogenesis.	bind
27474	2	8257	6	13	NULL	NULL	NULL	VEGF-D	GP	human	bind					VEGFR-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_4_1405_s_373	11943725	46  Human VEGF-D binds and activates VEGFR-2 and VEGFR-3, suggesting roles in angiogenesis and lymphangiogenesis.	bind
27475	3	8257	6	13	NULL	NULL	NULL	statement 1	Process		activates					VEGFR-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_4_1405_s_373	11943725	46  Human VEGF-D binds and activates VEGFR-2 and VEGFR-3, suggesting roles in angiogenesis and lymphangiogenesis.	bind
27476	4	8257	6	13	NULL	NULL	NULL	statement 2	Process		activates					VEGFR-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_4_1405_s_373	11943725	46  Human VEGF-D binds and activates VEGFR-2 and VEGFR-3, suggesting roles in angiogenesis and lymphangiogenesis.	bind
27477	5	8257	6	13	NULL	NULL	NULL	statement 1	Process		plays a role in					angiogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_4_1405_s_373	11943725	46  Human VEGF-D binds and activates VEGFR-2 and VEGFR-3, suggesting roles in angiogenesis and lymphangiogenesis.	bind
27478	6	8257	6	13	NULL	NULL	NULL	statement 2	Process		plays a role in					lymphangiogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_4_1405_s_373	11943725	46  Human VEGF-D binds and activates VEGFR-2 and VEGFR-3, suggesting roles in angiogenesis and lymphangiogenesis.	bind
33498	1	8257	7	NULL	NULL	0	NULL	VEGF-D	NULL	human	binds	NULL				VEGFR-2	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_4_1405_s_373	11943725	46  Human VEGF-D binds and activates VEGFR-2 and VEGFR-3, suggesting roles in angiogenesis and lymphangiogenesis.	bind
33499	2	8257	7	10	NULL	0	NULL	VEGF-D	NULL	human	binds	NULL				VEGFR-3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_4_1405_s_373	11943725	46  Human VEGF-D binds and activates VEGFR-2 and VEGFR-3, suggesting roles in angiogenesis and lymphangiogenesis.	bind
33500	3	8257	7	NULL	NULL	0	NULL	statement 1	NULL		activates	NULL				VEGFR-2	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_4_1405_s_373	11943725	46  Human VEGF-D binds and activates VEGFR-2 and VEGFR-3, suggesting roles in angiogenesis and lymphangiogenesis.	bind
33501	4	8257	7	NULL	NULL	0	NULL	statement 2	NULL		activates	NULL				VEGFR-3	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_4_1405_s_373	11943725	46  Human VEGF-D binds and activates VEGFR-2 and VEGFR-3, suggesting roles in angiogenesis and lymphangiogenesis.	bind
33502	5	8257	7	10	NULL	0	NULL	statement 1			plays a role in					angiogenesis					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_4_1405_s_373	11943725	46  Human VEGF-D binds and activates VEGFR-2 and VEGFR-3, suggesting roles in angiogenesis and lymphangiogenesis.	bind
33503	6	8257	7	10	NULL	0	NULL	statement 2			plays a role in					lymphangiogenesis					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_4_1405_s_373	11943725	46  Human VEGF-D binds and activates VEGFR-2 and VEGFR-3, suggesting roles in angiogenesis and lymphangiogenesis.	bind
27479	1	8258	6	13	NULL	NULL	NULL	Lp(a)	GP		bind					THP-1 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2036_s_210	9351369	46  Therefore, binding of either Lp(a) or plasminogen to THP-1 cells will be the result of interactions governed by their relative affinities and concentrations.	bind
27480	2	8258	6	13	NULL	NULL	NULL	plasminogen	GP		bind					THP-1 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2036_s_210	9351369	46  Therefore, binding of either Lp(a) or plasminogen to THP-1 cells will be the result of interactions governed by their relative affinities and concentrations.	bind
27481	3	8258	6	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2036_s_210	9351369	46  Therefore, binding of either Lp(a) or plasminogen to THP-1 cells will be the result of interactions governed by their relative affinities and concentrations.	bind
33504	1	8258	7	NULL	NULL	0	NULL	Lp(a)	NULL		bind	NULL				THP-1 cells	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2036_s_210	9351369	46  Therefore, binding of either Lp(a) or plasminogen to THP-1 cells will be the result of interactions governed by their relative affinities and concentrations.	bind
33505	2	8258	7	NULL	NULL	0	NULL	plasminogen	NULL		bind	NULL				THP-1 cells	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2036_s_210	9351369	46  Therefore, binding of either Lp(a) or plasminogen to THP-1 cells will be the result of interactions governed by their relative affinities and concentrations.	bind
46801	3	8258	7	10	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2036_s_210	9351369	46  Therefore, binding of either Lp(a) or plasminogen to THP-1 cells will be the result of interactions governed by their relative affinities and concentrations.	bind
27482	1	8259	6	13	NULL	NULL	NULL	vWF	GP		bind					GPIb	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_6_793_s_194	7773736	46  This agglutination is ADP dependent and is the result of the binding of vWF to both the GPIb and GPIIb/IIIa complexes.	bind
27483	2	8259	6	13	NULL	NULL	NULL	vWF	GP		bind					GPIIb/IIIa complexes	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_6_793_s_194	7773736	46  This agglutination is ADP dependent and is the result of the binding of vWF to both the GPIb and GPIIb/IIIa complexes.	bind
27484	3	8259	6	13	NULL	NULL	NULL	statement 1	Process		occurs simultaneously with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_6_793_s_194	7773736	46  This agglutination is ADP dependent and is the result of the binding of vWF to both the GPIb and GPIIb/IIIa complexes.	bind
27485	4	8259	6	13	NULL	NULL	NULL	statement 3	Process		results in					agglutination	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_6_793_s_194	7773736	46  This agglutination is ADP dependent and is the result of the binding of vWF to both the GPIb and GPIIb/IIIa complexes.	bind
27486	5	8259	6	13	NULL	NULL	NULL	statement 4	Process		is dependent on					ADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_6_793_s_194	7773736	46  This agglutination is ADP dependent and is the result of the binding of vWF to both the GPIb and GPIIb/IIIa complexes.	bind
33506	1	8259	7	NULL	NULL	0	NULL	vWF	NULL		bind	NULL				GPIb 	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_6_793_s_194	7773736	46  This agglutination is ADP dependent and is the result of the binding of vWF to both the GPIb and GPIIb/IIIa complexes.	bind
33507	2	8259	7	NULL	NULL	0	NULL	vWF	NULL		bind	NULL				GPIIb/IIIa complex	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_6_793_s_194	7773736	46  This agglutination is ADP dependent and is the result of the binding of vWF to both the GPIb and GPIIb/IIIa complexes.	bind
33508	3	8259	7	10	NULL	0	NULL	statement 1	NULL		occurs simultaneously with	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_6_793_s_194	7773736	46  This agglutination is ADP dependent and is the result of the binding of vWF to both the GPIb and GPIIb/IIIa complexes.	bind
33509	4	8259	7	10	NULL	0	NULL	statement 3	NULL		results in	NULL				agglutination	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_6_793_s_194	7773736	46  This agglutination is ADP dependent and is the result of the binding of vWF to both the GPIb and GPIIb/IIIa complexes.	bind
33510	5	8259	7	10	NULL	0	NULL	statement 4	NULL		is dependent on	NULL				ADP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_6_793_s_194	7773736	46  This agglutination is ADP dependent and is the result of the binding of vWF to both the GPIb and GPIIb/IIIa complexes.	bind
27487	1	8260	6	13	NULL	NULL	NULL	VEGF121	GP		does not bind					neuropilins	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_14_1887_s_162	11294808	46  VEGF121 is a secreted isoform that lacks the heparin-binding domain; it does not bind to neuropilins.	bind
27488	2	8260	6	13	NULL	NULL	NULL	VEGF121	GP		lacks								heparin binding domain		NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_14_1887_s_162	11294808	46  VEGF121 is a secreted isoform that lacks the heparin-binding domain; it does not bind to neuropilins.	bind
46802	3	8260	6	13	NULL	NULL	NULL	VEGF121	GP		is a type of					secreted isoform	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_14_1887_s_162	11294808	46  VEGF121 is a secreted isoform that lacks the heparin-binding domain; it does not bind to neuropilins.	bind
33511	1	8260	7	NULL	NULL	0	NULL	VEGF121	NULL		is a type of	NULL				secreted isoform	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_14_1887_s_162	11294808	46  VEGF121 is a secreted isoform that lacks the heparin-binding domain; it does not bind to neuropilins.	bind
33512	2	8260	7	NULL	NULL	0	NULL	VEGF121	NULL		lacks	NULL					NULL		heparin-binding domain		NULL		0	NULL	NULL	NULL	gw60_circulation_103_14_1887_s_162	11294808	46  VEGF121 is a secreted isoform that lacks the heparin-binding domain; it does not bind to neuropilins.	bind
33513	3	8260	7	NULL	NULL	0	NULL	VEGF121	NULL		does not bind	NULL				neuropilins	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_14_1887_s_162	11294808	46  VEGF121 is a secreted isoform that lacks the heparin-binding domain; it does not bind to neuropilins.	bind
27489	1	8261	6	13	NULL	NULL	NULL	large LDL particles	GP	apo E-enriched	bind					chondroitin sulfate PGs	GP	arterial			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1216_s_181	9261249	46 47  Previously, we showed that large, apo E-enriched LDL particles preferentially bind to arterial chondroitin sulfate PGs in vitro compared with small, apo E-poor LDL particles, and part of the increased binding was related to the apo E content of the LDL. 16 17  In addition, we have shown that apo E is responsible for an increased binding affinity of large LDL particles from cynomolgus monkeys to fibroblasts in culture.	bind
27490	2	8261	6	13	NULL	NULL	NULL	small LDL particles	GP	apo E-poor	bind					chondroitin sulfate PGs	GP	arterial			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1216_s_181	9261249	46 47  Previously, we showed that large, apo E-enriched LDL particles preferentially bind to arterial chondroitin sulfate PGs in vitro compared with small, apo E-poor LDL particles, and part of the increased binding was related to the apo E content of the LDL. 16 17  In addition, we have shown that apo E is responsible for an increased binding affinity of large LDL particles from cynomolgus monkeys to fibroblasts in culture.	bind
27491	3	8261	6	13	NULL	NULL	NULL	statement 1	Process		is more preferential than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1216_s_181	9261249	46 47  Previously, we showed that large, apo E-enriched LDL particles preferentially bind to arterial chondroitin sulfate PGs in vitro compared with small, apo E-poor LDL particles, and part of the increased binding was related to the apo E content of the LDL. 16 17  In addition, we have shown that apo E is responsible for an increased binding affinity of large LDL particles from cynomolgus monkeys to fibroblasts in culture.	bind
27492	4	8261	6	13	NULL	NULL	NULL	large LDL particles	GP	cynomolgus monkeys	bind					fibroblasts	Cell				NULL	culture	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1216_s_181	9261249	46 47  Previously, we showed that large, apo E-enriched LDL particles preferentially bind to arterial chondroitin sulfate PGs in vitro compared with small, apo E-poor LDL particles, and part of the increased binding was related to the apo E content of the LDL. 16 17  In addition, we have shown that apo E is responsible for an increased binding affinity of large LDL particles from cynomolgus monkeys to fibroblasts in culture.	bind
27493	5	8261	6	13	NULL	NULL	NULL	apoE	GP		is responsible for					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1216_s_181	9261249	46 47  Previously, we showed that large, apo E-enriched LDL particles preferentially bind to arterial chondroitin sulfate PGs in vitro compared with small, apo E-poor LDL particles, and part of the increased binding was related to the apo E content of the LDL. 16 17  In addition, we have shown that apo E is responsible for an increased binding affinity of large LDL particles from cynomolgus monkeys to fibroblasts in culture.	bind
33524	1	8261	7	10	NULL	0	NULL	large LDL particles 	NULL	apo E-enriched	binds	NULL	preferentially			chondroitin sulfate PGs	NULL	arterial			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1216_s_181	9261249	46 47  Previously, we showed that large, apo E-enriched LDL particles preferentially bind to arterial chondroitin sulfate PGs in vitro compared with small, apo E-poor LDL particles, and part of the increased binding was related to the apo E content of the LDL. 16 17  In addition, we have shown that apo E is responsible for an increased binding affinity of large LDL particles from cynomolgus monkeys to fibroblasts in culture.	bind
33525	2	8261	7	10	NULL	0	NULL	small LDL particles	NULL	apo E-poor	bind	NULL				chondroitin sulfate PGs	NULL	arterial			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1216_s_181	9261249	46 47  Previously, we showed that large, apo E-enriched LDL particles preferentially bind to arterial chondroitin sulfate PGs in vitro compared with small, apo E-poor LDL particles, and part of the increased binding was related to the apo E content of the LDL. 16 17  In addition, we have shown that apo E is responsible for an increased binding affinity of large LDL particles from cynomolgus monkeys to fibroblasts in culture.	bind
33526	3	8261	7	NULL	NULL	0	NULL	statement 1	NULL		is preferred over	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1216_s_181	9261249	46 47  Previously, we showed that large, apo E-enriched LDL particles preferentially bind to arterial chondroitin sulfate PGs in vitro compared with small, apo E-poor LDL particles, and part of the increased binding was related to the apo E content of the LDL. 16 17  In addition, we have shown that apo E is responsible for an increased binding affinity of large LDL particles from cynomolgus monkeys to fibroblasts in culture.	bind
33527	4	8261	7	10	NULL	0	NULL	statement 3	NULL		is related to	NULL				LDL	NULL	apo E content of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1216_s_181	9261249	46 47  Previously, we showed that large, apo E-enriched LDL particles preferentially bind to arterial chondroitin sulfate PGs in vitro compared with small, apo E-poor LDL particles, and part of the increased binding was related to the apo E content of the LDL. 16 17  In addition, we have shown that apo E is responsible for an increased binding affinity of large LDL particles from cynomolgus monkeys to fibroblasts in culture.	bind
33528	5	8261	7	NULL	NULL	0	NULL	large LDL particles	NULL	cynomolgus monkeys	bind	NULL				fibroblasts	NULL				NULL	in culture	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1216_s_181	9261249	46 47  Previously, we showed that large, apo E-enriched LDL particles preferentially bind to arterial chondroitin sulfate PGs in vitro compared with small, apo E-poor LDL particles, and part of the increased binding was related to the apo E content of the LDL. 16 17  In addition, we have shown that apo E is responsible for an increased binding affinity of large LDL particles from cynomolgus monkeys to fibroblasts in culture.	bind
33529	6	8261	7	NULL	NULL	0	NULL	apo E	NULL		increase	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1216_s_181	9261249	46 47  Previously, we showed that large, apo E-enriched LDL particles preferentially bind to arterial chondroitin sulfate PGs in vitro compared with small, apo E-poor LDL particles, and part of the increased binding was related to the apo E content of the LDL. 16 17  In addition, we have shown that apo E is responsible for an increased binding affinity of large LDL particles from cynomolgus monkeys to fibroblasts in culture.	bind
27494	1	8262	6	13	NULL	NULL	NULL	LXR/RXR heterodimer	GP	activated;; nuclear	bind									DR4 element of promoter	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_10_1535_s_82	12377728	46 Expression of this gene is regulated by activated liver X receptor (LXR)/retinoid X receptor (RXR) nuclear heterodimers that bind to the DR4 element in its promoter region.	bind
27495	2	8262	6	13	NULL	NULL	NULL	LXR	GP		is					liver X receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_10_1535_s_82	12377728	46 Expression of this gene is regulated by activated liver X receptor (LXR)/retinoid X receptor (RXR) nuclear heterodimers that bind to the DR4 element in its promoter region.	bind
27496	3	8262	6	13	NULL	NULL	NULL	RXR	GP		is					retinoid X receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_10_1535_s_82	12377728	46 Expression of this gene is regulated by activated liver X receptor (LXR)/retinoid X receptor (RXR) nuclear heterodimers that bind to the DR4 element in its promoter region.	bind
33530	1	8262	7	10	NULL	0	NULL	LXR/RXR heterodimer	NULL	activated;;nuclear	binds to	NULL					NULL			DR4 element in the promoter	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_10_1535_s_82	12377728	46 Expression of this gene is regulated by activated liver X receptor (LXR)/retinoid X receptor (RXR) nuclear heterodimers that bind to the DR4 element in its promoter region.	bind
33531	2	8262	7	NULL	NULL	0	NULL	LXR	NULL		is	NULL				liver X receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_10_1535_s_82	12377728	46 Expression of this gene is regulated by activated liver X receptor (LXR)/retinoid X receptor (RXR) nuclear heterodimers that bind to the DR4 element in its promoter region.	bind
33532	3	8262	7	NULL	NULL	0	NULL	RXR	NULL		is	NULL				retinoid X receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_10_1535_s_82	12377728	46 Expression of this gene is regulated by activated liver X receptor (LXR)/retinoid X receptor (RXR) nuclear heterodimers that bind to the DR4 element in its promoter region.	bind
27497	1	8263	6	13	NULL	NULL	NULL	SMemb gene	GP		bind				KLF5-binding element	Sp1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1135_s_100	15817882	46 We have also shown that the KLF5-binding element in the SMemb gene also binds Sp1 in vitro.	bind
33533	1	8263	7	NULL	NULL	0	NULL	SMemb gene	NULL		binds	NULL			KLF5-binding element	Sp1	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1135_s_100	15817882	46 We have also shown that the KLF5-binding element in the SMemb gene also binds Sp1 in vitro.	bind
27498	1	8264	6	13	NULL	NULL	NULL	MCs	Cell	cultured	bind					IL12	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_2_623_s_257	10027419	46, 47  erein, we demonstrate that cultured MCs bind IL-12 and express the human low-affinity IL-12 beta1 chain receptor under basal conditions.	bind
27499	2	8264	6	13	NULL	NULL	NULL	MCs	Cell	cultured	express					IL-12 beta1 chain receptor	GP	human;; low affinity			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_2_623_s_257	10027419	46, 47  erein, we demonstrate that cultured MCs bind IL-12 and express the human low-affinity IL-12 beta1 chain receptor under basal conditions.	bind
33534	1	8264	7	10	NULL	0	NULL	MCs	NULL	cultured	bind	NULL				IL-12	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_2_623_s_257	10027419	46, 47  erein, we demonstrate that cultured MCs bind IL-12 and express the human low-affinity IL-12 beta1 chain receptor under basal conditions.	bind
33535	2	8264	7	10	NULL	0	NULL	MCs	NULL	cultured	express	NULL				IL-12 beta1 chain receptor	NULL	human;;low-affinity			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_2_623_s_257	10027419	46, 47  erein, we demonstrate that cultured MCs bind IL-12 and express the human low-affinity IL-12 beta1 chain receptor under basal conditions.	bind
27500	1	8265	6	13	NULL	NULL	NULL	VEGF-E	GP		bind		exclusively			VEGFR-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1143_s_116	12676799	46,47  Because infusion of VEGF-E, which binds exclusively to VEGFR-2, did not influence arteriogenesis, we concluded that the effects of VEGF-A on arteriogenesis are caused by monocyte activation.	bind
27501	2	8265	6	13	NULL	NULL	NULL	statement 1	Process		did not influence					arteriogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1143_s_116	12676799	46,47  Because infusion of VEGF-E, which binds exclusively to VEGFR-2, did not influence arteriogenesis, we concluded that the effects of VEGF-A on arteriogenesis are caused by monocyte activation.	bind
27502	4	8265	6	13	NULL	NULL	NULL	monocyte	Cell	activation of	causes					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1143_s_116	12676799	46,47  Because infusion of VEGF-E, which binds exclusively to VEGFR-2, did not influence arteriogenesis, we concluded that the effects of VEGF-A on arteriogenesis are caused by monocyte activation.	bind
46803	3	8265	6	13	NULL	NULL	NULL	VEGF-A 	GP		effects					arteriogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1143_s_116	12676799	46,47  Because infusion of VEGF-E, which binds exclusively to VEGFR-2, did not influence arteriogenesis, we concluded that the effects of VEGF-A on arteriogenesis are caused by monocyte activation.	bind
33536	1	8265	7	NULL	NULL	0	NULL	VEGF-E	NULL		binds	NULL	exclusively			VEGFR-2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1143_s_116	12676799	46,47  Because infusion of VEGF-E, which binds exclusively to VEGFR-2, did not influence arteriogenesis, we concluded that the effects of VEGF-A on arteriogenesis are caused by monocyte activation.	bind
33537	2	8265	7	NULL	NULL	0	NULL	statement 1	NULL		does not influence	NULL				arteriogenesis	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1143_s_116	12676799	46,47  Because infusion of VEGF-E, which binds exclusively to VEGFR-2, did not influence arteriogenesis, we concluded that the effects of VEGF-A on arteriogenesis are caused by monocyte activation.	bind
33541	3	8265	7	NULL	NULL	0	NULL	VEGF-A	NULL		effects	NULL				arteriogenesis	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1143_s_116	12676799	46,47  Because infusion of VEGF-E, which binds exclusively to VEGFR-2, did not influence arteriogenesis, we concluded that the effects of VEGF-A on arteriogenesis are caused by monocyte activation.	bind
33543	4	8265	7	10	NULL	0	NULL	monocyte	NULL	activation of	causes	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1143_s_116	12676799	46,47  Because infusion of VEGF-E, which binds exclusively to VEGFR-2, did not influence arteriogenesis, we concluded that the effects of VEGF-A on arteriogenesis are caused by monocyte activation.	bind
27561	1	8266	6	13	NULL	NULL	NULL	PECAM-1 	GP		is required for			ITIM		SHP-1	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_69	12689916	46,50,57 - 59      As with SHP-2, both PECAM-1 ITIMs seem to be required to support SHP-1 binding 50; however, unlike SHP-2, the affinity between SHP-1 and pY663 is identical to that of pY686, and the affinities of both interactions are significantly lower than those reported for SHP-2.	bind
27562	2	8266	6	13	NULL	NULL	NULL	PECAM-1	GP		is required for			ITIM		SHP-2	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_69	12689916	46,50,57 - 59      As with SHP-2, both PECAM-1 ITIMs seem to be required to support SHP-1 binding 50; however, unlike SHP-2, the affinity between SHP-1 and pY663 is identical to that of pY686, and the affinities of both interactions are significantly lower than those reported for SHP-2.	bind
27563	3	8266	6	13	NULL	NULL	NULL	SHP-1	GP		interacts with								pY663		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_69	12689916	46,50,57 - 59      As with SHP-2, both PECAM-1 ITIMs seem to be required to support SHP-1 binding 50; however, unlike SHP-2, the affinity between SHP-1 and pY663 is identical to that of pY686, and the affinities of both interactions are significantly lower than those reported for SHP-2.	bind
27564	4	8266	6	13	NULL	NULL	NULL	SHP-1	GP		interacts with								pY686		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_69	12689916	46,50,57 - 59      As with SHP-2, both PECAM-1 ITIMs seem to be required to support SHP-1 binding 50; however, unlike SHP-2, the affinity between SHP-1 and pY663 is identical to that of pY686, and the affinities of both interactions are significantly lower than those reported for SHP-2.	bind
27565	5	8266	6	13	NULL	NULL	NULL	statement 3	Process	affinity of	is equal to					statement 4	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_69	12689916	46,50,57 - 59      As with SHP-2, both PECAM-1 ITIMs seem to be required to support SHP-1 binding 50; however, unlike SHP-2, the affinity between SHP-1 and pY663 is identical to that of pY686, and the affinities of both interactions are significantly lower than those reported for SHP-2.	bind
27566	6	8266	6	13	NULL	NULL	NULL	SHP-2	GP		interacts with								pY663		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_69	12689916	46,50,57 - 59      As with SHP-2, both PECAM-1 ITIMs seem to be required to support SHP-1 binding 50; however, unlike SHP-2, the affinity between SHP-1 and pY663 is identical to that of pY686, and the affinities of both interactions are significantly lower than those reported for SHP-2.	bind
27567	7	8266	6	13	NULL	NULL	NULL	SHP-2	GP		interacts with								pY686		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_69	12689916	46,50,57 - 59      As with SHP-2, both PECAM-1 ITIMs seem to be required to support SHP-1 binding 50; however, unlike SHP-2, the affinity between SHP-1 and pY663 is identical to that of pY686, and the affinities of both interactions are significantly lower than those reported for SHP-2.	bind
27568	8	8266	6	13	NULL	NULL	NULL	statement 3	Process	affinity of	is lower than		significantly			statement 6	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_69	12689916	46,50,57 - 59      As with SHP-2, both PECAM-1 ITIMs seem to be required to support SHP-1 binding 50; however, unlike SHP-2, the affinity between SHP-1 and pY663 is identical to that of pY686, and the affinities of both interactions are significantly lower than those reported for SHP-2.	bind
27569	9	8266	6	13	NULL	NULL	NULL	statement 4	Process	affinity of	is lower than		significantly			statement 7	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_69	12689916	46,50,57 - 59      As with SHP-2, both PECAM-1 ITIMs seem to be required to support SHP-1 binding 50; however, unlike SHP-2, the affinity between SHP-1 and pY663 is identical to that of pY686, and the affinities of both interactions are significantly lower than those reported for SHP-2.	bind
33545	1	8266	7	10	NULL	0	NULL	PECAM-1	NULL		support	NULL		ITIMs		SHP-1	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_69	12689916	46,50,57 - 59      As with SHP-2, both PECAM-1 ITIMs seem to be required to support SHP-1 binding 50; however, unlike SHP-2, the affinity between SHP-1 and pY663 is identical to that of pY686, and the affinities of both interactions are significantly lower than those reported for SHP-2.	bind
33547	2	8266	7	10	NULL	0	NULL	PECAM-1	NULL		support	NULL		ITIMs		SHP-2	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_69	12689916	46,50,57 - 59      As with SHP-2, both PECAM-1 ITIMs seem to be required to support SHP-1 binding 50; however, unlike SHP-2, the affinity between SHP-1 and pY663 is identical to that of pY686, and the affinities of both interactions are significantly lower than those reported for SHP-2.	bind
33549	3	8266	7	NULL	NULL	0	NULL	SHP-1	NULL		bind	NULL					NULL		pY663		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_69	12689916	46,50,57 - 59      As with SHP-2, both PECAM-1 ITIMs seem to be required to support SHP-1 binding 50; however, unlike SHP-2, the affinity between SHP-1 and pY663 is identical to that of pY686, and the affinities of both interactions are significantly lower than those reported for SHP-2.	bind
33550	4	8266	7	NULL	NULL	0	NULL	SHP-1	NULL		bind	NULL					NULL		pY686		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_69	12689916	46,50,57 - 59      As with SHP-2, both PECAM-1 ITIMs seem to be required to support SHP-1 binding 50; however, unlike SHP-2, the affinity between SHP-1 and pY663 is identical to that of pY686, and the affinities of both interactions are significantly lower than those reported for SHP-2.	bind
33554	5	8266	7	NULL	NULL	0	NULL	statement 3	NULL	affinity of	is identical to	NULL				statement 4	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_69	12689916	46,50,57 - 59      As with SHP-2, both PECAM-1 ITIMs seem to be required to support SHP-1 binding 50; however, unlike SHP-2, the affinity between SHP-1 and pY663 is identical to that of pY686, and the affinities of both interactions are significantly lower than those reported for SHP-2.	bind
33557	6	8266	7	NULL	NULL	0	NULL	 SHP-2	NULL		bind	NULL					NULL		pY663		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_69	12689916	46,50,57 - 59      As with SHP-2, both PECAM-1 ITIMs seem to be required to support SHP-1 binding 50; however, unlike SHP-2, the affinity between SHP-1 and pY663 is identical to that of pY686, and the affinities of both interactions are significantly lower than those reported for SHP-2.	bind
33560	7	8266	7	NULL	NULL	0	NULL	SHP-2	NULL		bind	NULL					NULL		pY686		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_69	12689916	46,50,57 - 59      As with SHP-2, both PECAM-1 ITIMs seem to be required to support SHP-1 binding 50; however, unlike SHP-2, the affinity between SHP-1 and pY663 is identical to that of pY686, and the affinities of both interactions are significantly lower than those reported for SHP-2.	bind
46804	8	8266	7	10	NULL	0	NULL	statement 3	NULL	affinity of	is lower than	NULL	significantly			statement 6	NULL	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_69	12689916	46,50,57 - 59      As with SHP-2, both PECAM-1 ITIMs seem to be required to support SHP-1 binding 50; however, unlike SHP-2, the affinity between SHP-1 and pY663 is identical to that of pY686, and the affinities of both interactions are significantly lower than those reported for SHP-2.	bind
46806	9	8266	7	10	NULL	0	NULL	statement 4	NULL	affinity of	is lower than	NULL	significantly			statement 7	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_6_953_s_69	12689916	46,50,57 - 59      As with SHP-2, both PECAM-1 ITIMs seem to be required to support SHP-1 binding 50; however, unlike SHP-2, the affinity between SHP-1 and pY663 is identical to that of pY686, and the affinities of both interactions are significantly lower than those reported for SHP-2.	bind
27503	1	8267	6	13	NULL	NULL	NULL	hypoxia	MedicalFinding		decreases					TGF-beta1 receptor	GP	binding of			NULL	dermal fibroblasts	NULL	NULL	NULL	NULL	gw60_amjpathol_154_1_301_s_193	9916944	46- 48  It was also reported that hypoxia decreases TGF-beta1 receptor binding and synthesis in dermal fibroblasts.	bind
27504	2	8267	6	13	NULL	NULL	NULL	hypoxia	MedicalFinding		decreases					TGF-beta1 receptor	GP	synthesis of			NULL	dermal fibroblasts	NULL	NULL	NULL	NULL	gw60_amjpathol_154_1_301_s_193	9916944	46- 48  It was also reported that hypoxia decreases TGF-beta1 receptor binding and synthesis in dermal fibroblasts.	bind
33567	1	8267	7	10	NULL	0	NULL	hypoxia 			decrease					TGF-beta1 receptor		binding of			NULL	dermal fibroblasts	NULL	NULL	NULL	NULL	gw60_amjpathol_154_1_301_s_193	9916944	46- 48  It was also reported that hypoxia decreases TGF-beta1 receptor binding and synthesis in dermal fibroblasts.	bind
33572	2	8267	7	NULL	NULL	0	NULL	hypoxia	NULL		decrease	NULL				TGF-beta1 receptor	NULL	synthesis of			NULL	dermal fibroblasts	NULL	NULL	NULL	NULL	gw60_amjpathol_154_1_301_s_193	9916944	46- 48  It was also reported that hypoxia decreases TGF-beta1 receptor binding and synthesis in dermal fibroblasts.	bind
27505	1	8268	6	13	NULL	NULL	NULL	LDL	GP		does not bind					GPIIb-IIIa complex	GP				NULL	intact resting platelets	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_156_s_188	9012651	47  In conclusion, we present ample evidence indicating that neither the GPIIb-IIIa complex nor GPIIb and GPIIIa individually are the ligand binding proteins for LDL on intact resting platelets.	bind
27506	2	8268	6	13	NULL	NULL	NULL	LDL	GP		does not bind					GPIIb	GP				NULL	intact resting platelets	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_156_s_188	9012651	47  In conclusion, we present ample evidence indicating that neither the GPIIb-IIIa complex nor GPIIb and GPIIIa individually are the ligand binding proteins for LDL on intact resting platelets.	bind
27507	3	8268	6	13	NULL	NULL	NULL	LDL	GP		does not bind					GPIIIa	GP				NULL	intact resting platelets	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_156_s_188	9012651	47  In conclusion, we present ample evidence indicating that neither the GPIIb-IIIa complex nor GPIIb and GPIIIa individually are the ligand binding proteins for LDL on intact resting platelets.	bind
33579	1	8268	7	NULL	NULL	0	NULL	GPIIb-IIIa complex 	NULL		does not bind	NULL				LDL	NULL				NULL	intact resting platelets	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_156_s_188	9012651	47  In conclusion, we present ample evidence indicating that neither the GPIIb-IIIa complex nor GPIIb and GPIIIa individually are the ligand binding proteins for LDL on intact resting platelets.	bind
33580	2	8268	7	NULL	NULL	0	NULL	GPIIb	NULL		does not bind	NULL				LDL	NULL				NULL	intact resting platelets	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_156_s_188	9012651	47  In conclusion, we present ample evidence indicating that neither the GPIIb-IIIa complex nor GPIIb and GPIIIa individually are the ligand binding proteins for LDL on intact resting platelets.	bind
33751	3	8268	7	NULL	NULL	0	NULL	GPIIIa	NULL		does not bind	NULL				LDL	NULL				NULL	intact resting platelets	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_156_s_188	9012651	47  In conclusion, we present ample evidence indicating that neither the GPIIb-IIIa complex nor GPIIb and GPIIIa individually are the ligand binding proteins for LDL on intact resting platelets.	bind
27570	1	8269	6	13	NULL	NULL	NULL	FGF-2	GP		bind					FGFR-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_185_s_302	11786412	47  Interestingly, 6-O sulfate on glucosamine is the main structural feature within HS GAGs required to promote binding of FGF-2 to FGFR-1 and to stimulate signaling.	bind
28330	2	8269	6	13	NULL	NULL	NULL	HS GAGs	GP		contains					6-O sulfate on glucosamine	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_185_s_302	11786412	47  Interestingly, 6-O sulfate on glucosamine is the main structural feature within HS GAGs required to promote binding of FGF-2 to FGFR-1 and to stimulate signaling.	bind
28331	3	8269	6	13	NULL	NULL	NULL	statement 2	Process		is required for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_185_s_302	11786412	47  Interestingly, 6-O sulfate on glucosamine is the main structural feature within HS GAGs required to promote binding of FGF-2 to FGFR-1 and to stimulate signaling.	bind
28332	4	8269	6	13	NULL	NULL	NULL	statement 2	Process		stimulates					signaling	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_185_s_302	11786412	47  Interestingly, 6-O sulfate on glucosamine is the main structural feature within HS GAGs required to promote binding of FGF-2 to FGFR-1 and to stimulate signaling.	bind
33752	1	8269	7	NULL	NULL	0	NULL	FGF-2	NULL		bind	NULL				 FGFR-1	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_1_185_s_302	11786412	47  Interestingly, 6-O sulfate on glucosamine is the main structural feature within HS GAGs required to promote binding of FGF-2 to FGFR-1 and to stimulate signaling.	bind
33753	2	8269	7	NULL	NULL	0	NULL	6-O sulfate glucosamine	NULL		is present in	NULL				HS GAGs	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_185_s_302	11786412	47  Interestingly, 6-O sulfate on glucosamine is the main structural feature within HS GAGs required to promote binding of FGF-2 to FGFR-1 and to stimulate signaling.	bind
33754	3	8269	7	NULL	NULL	0	NULL	statement 2	NULL		promote	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_1_185_s_302	11786412	47  Interestingly, 6-O sulfate on glucosamine is the main structural feature within HS GAGs required to promote binding of FGF-2 to FGFR-1 and to stimulate signaling.	bind
33755	4	8269	7	NULL	NULL	0	NULL	statement 3	NULL		stimulate	NULL				signaling	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_1_185_s_302	11786412	47  Interestingly, 6-O sulfate on glucosamine is the main structural feature within HS GAGs required to promote binding of FGF-2 to FGFR-1 and to stimulate signaling.	bind
27571	1	8270	6	13	NULL	NULL	NULL	Lp(a)	GP		bind					fibrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_385_s_193	7749849	47  Much of the binding of Lp(a) by fibrin is lysine mediated, and as the present results show, the lysine-binding properties of Lp(a) are not affected by in vitro glycation as performed under these conditions.	bind
27572	2	8270	6	13	NULL	NULL	NULL	statement 1	Process		is mediated by					lysine	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_385_s_193	7749849	47  Much of the binding of Lp(a) by fibrin is lysine mediated, and as the present results show, the lysine-binding properties of Lp(a) are not affected by in vitro glycation as performed under these conditions.	bind
27573	3	8270	6	13	NULL	NULL	NULL	Lp(a)	GP		bind					lysine	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_385_s_193	7749849	47  Much of the binding of Lp(a) by fibrin is lysine mediated, and as the present results show, the lysine-binding properties of Lp(a) are not affected by in vitro glycation as performed under these conditions.	bind
27574	4	8270	6	13	NULL	NULL	NULL	statement 3	Process		is not affected by					glycation	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_385_s_193	7749849	47  Much of the binding of Lp(a) by fibrin is lysine mediated, and as the present results show, the lysine-binding properties of Lp(a) are not affected by in vitro glycation as performed under these conditions.	bind
33756	1	8270	7	NULL	NULL	0	NULL	fibrin 	NULL		bind	NULL				Lp(a)	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_385_s_193	7749849	47  Much of the binding of Lp(a) by fibrin is lysine mediated, and as the present results show, the lysine-binding properties of Lp(a) are not affected by in vitro glycation as performed under these conditions.	bind
33757	2	8270	7	NULL	NULL	0	NULL	lysine	NULL		mediates	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_385_s_193	7749849	47  Much of the binding of Lp(a) by fibrin is lysine mediated, and as the present results show, the lysine-binding properties of Lp(a) are not affected by in vitro glycation as performed under these conditions.	bind
33758	3	8270	7	10	NULL	0	NULL	Lp(a)	NULL		bind	NULL				lusine	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_385_s_193	7749849	47  Much of the binding of Lp(a) by fibrin is lysine mediated, and as the present results show, the lysine-binding properties of Lp(a) are not affected by in vitro glycation as performed under these conditions.	bind
46807	4	8270	7	10	NULL	0	NULL	statement 3	NULL		is not affected by	NULL				glycation	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_385_s_193	7749849	47  Much of the binding of Lp(a) by fibrin is lysine mediated, and as the present results show, the lysine-binding properties of Lp(a) are not affected by in vitro glycation as performed under these conditions.	bind
28333	1	8271	6	13	NULL	NULL	NULL	large VLDL	GP		contains					prothrombin	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_1_33_s_138	9445253	48  Bradley and Gianturco 27  reported that the large VLDLs that were separated from hypertriglyceridemic patients contained prothrombin, but not those of normal subjects; they also demonstrated that prothrombin can bind to plasma VLDLs in vitro at physiological concentrations of VLDLs, prothrombin, and calcium, whereas binding to LDLs and HDLs was negligible.	bind
28334	2	8271	6	13	NULL	NULL	NULL	statement 1	Process		occurs in					hypertriglyceridemia	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_1_33_s_138	9445253	48  Bradley and Gianturco 27  reported that the large VLDLs that were separated from hypertriglyceridemic patients contained prothrombin, but not those of normal subjects; they also demonstrated that prothrombin can bind to plasma VLDLs in vitro at physiological concentrations of VLDLs, prothrombin, and calcium, whereas binding to LDLs and HDLs was negligible.	bind
28336	3	8271	6	13	NULL	NULL	NULL	prothrombin	GP		bind					VLDL	GP	plasma			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_1_33_s_138	9445253	48  Bradley and Gianturco 27  reported that the large VLDLs that were separated from hypertriglyceridemic patients contained prothrombin, but not those of normal subjects; they also demonstrated that prothrombin can bind to plasma VLDLs in vitro at physiological concentrations of VLDLs, prothrombin, and calcium, whereas binding to LDLs and HDLs was negligible.	bind
28337	4	8271	6	13	NULL	NULL	NULL	prothrombin	GP		bind		negligibly			LDLs	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_1_33_s_138	9445253	48  Bradley and Gianturco 27  reported that the large VLDLs that were separated from hypertriglyceridemic patients contained prothrombin, but not those of normal subjects; they also demonstrated that prothrombin can bind to plasma VLDLs in vitro at physiological concentrations of VLDLs, prothrombin, and calcium, whereas binding to LDLs and HDLs was negligible.	bind
28338	5	8271	6	13	NULL	NULL	NULL	prothrombin	GP		bind		negligibly			HDLs	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_1_33_s_138	9445253	48  Bradley and Gianturco 27  reported that the large VLDLs that were separated from hypertriglyceridemic patients contained prothrombin, but not those of normal subjects; they also demonstrated that prothrombin can bind to plasma VLDLs in vitro at physiological concentrations of VLDLs, prothrombin, and calcium, whereas binding to LDLs and HDLs was negligible.	bind
34028	1	8271	7	10	NULL	0	NULL	 prothrombin			bind					VLDL		plasma			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_1_33_s_138	9445253	48  Bradley and Gianturco 27  reported that the large VLDLs that were separated from hypertriglyceridemic patients contained prothrombin, but not those of normal subjects; they also demonstrated that prothrombin can bind to plasma VLDLs in vitro at physiological concentrations of VLDLs, prothrombin, and calcium, whereas binding to LDLs and HDLs was negligible.	bind
34029	2	8271	7	NULL	NULL	0	NULL	prothrombin	NULL		bind	NULL	negligibly			LDL	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_1_33_s_138	9445253	48  Bradley and Gianturco 27  reported that the large VLDLs that were separated from hypertriglyceridemic patients contained prothrombin, but not those of normal subjects; they also demonstrated that prothrombin can bind to plasma VLDLs in vitro at physiological concentrations of VLDLs, prothrombin, and calcium, whereas binding to LDLs and HDLs was negligible.	bind
34030	3	8271	7	NULL	NULL	0	NULL	prothrombin	NULL		bind	NULL	negligibly			HDL	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_1_33_s_138	9445253	48  Bradley and Gianturco 27  reported that the large VLDLs that were separated from hypertriglyceridemic patients contained prothrombin, but not those of normal subjects; they also demonstrated that prothrombin can bind to plasma VLDLs in vitro at physiological concentrations of VLDLs, prothrombin, and calcium, whereas binding to LDLs and HDLs was negligible.	bind
47534	4	8271	7	10	NULL	0	NULL	large VLDL	NULL		contains	NULL				prothrombin	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_1_33_s_138	9445253	48  Bradley and Gianturco 27  reported that the large VLDLs that were separated from hypertriglyceridemic patients contained prothrombin, but not those of normal subjects; they also demonstrated that prothrombin can bind to plasma VLDLs in vitro at physiological concentrations of VLDLs, prothrombin, and calcium, whereas binding to LDLs and HDLs was negligible.	bind
47535	5	8271	7	10	NULL	0	NULL	statement 4	NULL		occurs in	NULL				hypertriglyceridemia	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_1_33_s_138	9445253	48  Bradley and Gianturco 27  reported that the large VLDLs that were separated from hypertriglyceridemic patients contained prothrombin, but not those of normal subjects; they also demonstrated that prothrombin can bind to plasma VLDLs in vitro at physiological concentrations of VLDLs, prothrombin, and calcium, whereas binding to LDLs and HDLs was negligible.	bind
27575	1	8272	6	13	NULL	NULL	NULL	FXa	GP	free	does not bind		efficiently			TFPI	GP	cellular			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2251_s_241	10479670	48  For ECs, where free FXa is not efficiently bound by cellular TFPI, 23  downregulation of TF .	bind
34031	1	8272	7	10	NULL	0	NULL	TFPI	NULL	cellular	does not bind	NULL	efficiently			FXa	NULL	free			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_9_2251_s_241	10479670	48  For ECs, where free FXa is not efficiently bound by cellular TFPI, 23  downregulation of TF .	bind
34722	1	8273	6	13	NULL	NULL	NULL	PMA	Chemical		does not affect					Sp1	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_377_s_231	10669633	48 49  In the present study, the binding affinity of Sp1 and Sp3 to the probe is not reproducibly affected by PMA.	bind
34723	2	8273	6	13	NULL	NULL	NULL	PMA	Chemical		does not affect					Sp3	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_377_s_231	10669633	48 49  In the present study, the binding affinity of Sp1 and Sp3 to the probe is not reproducibly affected by PMA.	bind
34032	1	8273	7	10	NULL	0	NULL	PMA	NULL		does not affect	NULL				Sp1	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_377_s_231	10669633	48 49  In the present study, the binding affinity of Sp1 and Sp3 to the probe is not reproducibly affected by PMA.	bind
34033	2	8273	7	10	NULL	0	NULL	PMA	NULL		does not affect	NULL				Sp3	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_377_s_231	10669633	48 49  In the present study, the binding affinity of Sp1 and Sp3 to the probe is not reproducibly affected by PMA.	bind
28339	1	8274	6	13	NULL	NULL	NULL	statement 8	Chromosome		controls		may;;selectively			SRF	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_148	15718508	48 As such, it is interesting to speculate that there may be SMC-lineage specific patterning of chromatin structure that selectively controls SRF binding and subsequent recruitment of myocardin to a very select subset of SMC marker genes but not growth response genes like c- fos or skeletal and cardiac multiple CArG-containing genes.	bind
28340	2	8274	6	13	NULL	NULL	NULL	statement 8	Process		control		may;;selectively			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_148	15718508	48 As such, it is interesting to speculate that there may be SMC-lineage specific patterning of chromatin structure that selectively controls SRF binding and subsequent recruitment of myocardin to a very select subset of SMC marker genes but not growth response genes like c- fos or skeletal and cardiac multiple CArG-containing genes.	bind
28341	3	8274	6	13	NULL	NULL	NULL	myocardin	GP		is recruited to					SMC marker gene	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_148	15718508	48 As such, it is interesting to speculate that there may be SMC-lineage specific patterning of chromatin structure that selectively controls SRF binding and subsequent recruitment of myocardin to a very select subset of SMC marker genes but not growth response genes like c- fos or skeletal and cardiac multiple CArG-containing genes.	bind
28343	4	8274	6	13	NULL	NULL	NULL	myocardin	GP		is not recruited to					c-fos	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_148	15718508	48 As such, it is interesting to speculate that there may be SMC-lineage specific patterning of chromatin structure that selectively controls SRF binding and subsequent recruitment of myocardin to a very select subset of SMC marker genes but not growth response genes like c- fos or skeletal and cardiac multiple CArG-containing genes.	bind
28344	5	8274	6	13	NULL	NULL	NULL	c-fos	GP		is a type of					growth response gene	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_148	15718508	48 As such, it is interesting to speculate that there may be SMC-lineage specific patterning of chromatin structure that selectively controls SRF binding and subsequent recruitment of myocardin to a very select subset of SMC marker genes but not growth response genes like c- fos or skeletal and cardiac multiple CArG-containing genes.	bind
28346	6	8274	6	13	NULL	NULL	NULL	myocardin	GP		is not recruited to					multiple CArG-containing genes	GP	skeletal			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_148	15718508	48 As such, it is interesting to speculate that there may be SMC-lineage specific patterning of chromatin structure that selectively controls SRF binding and subsequent recruitment of myocardin to a very select subset of SMC marker genes but not growth response genes like c- fos or skeletal and cardiac multiple CArG-containing genes.	bind
47518	7	8274	6	13	NULL	NULL	NULL	myocardin	GP		is not recruited to					multiple CArG-containing genes	GP	cardiac			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_148	15718508	48 As such, it is interesting to speculate that there may be SMC-lineage specific patterning of chromatin structure that selectively controls SRF binding and subsequent recruitment of myocardin to a very select subset of SMC marker genes but not growth response genes like c- fos or skeletal and cardiac multiple CArG-containing genes.	bind
56109	8	8274	6	13	NULL	NULL	NULL	chromatin	Chromosome	patterning of;;structure of	specific to					SMC-lineage	Cell				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_148	15718508	48 As such, it is interesting to speculate that there may be SMC-lineage specific patterning of chromatin structure that selectively controls SRF binding and subsequent recruitment of myocardin to a very select subset of SMC marker genes but not growth response genes like c- fos or skeletal and cardiac multiple CArG-containing genes.	bind
56111	9	8274	6	13	NULL	NULL	NULL	statement 8	Chromosome		controls		may;;selectively			statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_148	15718508	48 As such, it is interesting to speculate that there may be SMC-lineage specific patterning of chromatin structure that selectively controls SRF binding and subsequent recruitment of myocardin to a very select subset of SMC marker genes but not growth response genes like c- fos or skeletal and cardiac multiple CArG-containing genes.	bind
56112	10	8274	6	13	NULL	NULL	NULL	statement 8	Chromosome		controls		may;;selectively			statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_148	15718508	48 As such, it is interesting to speculate that there may be SMC-lineage specific patterning of chromatin structure that selectively controls SRF binding and subsequent recruitment of myocardin to a very select subset of SMC marker genes but not growth response genes like c- fos or skeletal and cardiac multiple CArG-containing genes.	bind
56113	11	8274	6	13	NULL	NULL	NULL	statement 8	Chromosome		controls		may;;selectively			statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_148	15718508	48 As such, it is interesting to speculate that there may be SMC-lineage specific patterning of chromatin structure that selectively controls SRF binding and subsequent recruitment of myocardin to a very select subset of SMC marker genes but not growth response genes like c- fos or skeletal and cardiac multiple CArG-containing genes.	bind
34038	1	8274	7	NULL	NULL	0	NULL	myocardin	NULL		is recruited to	NULL				SMC marker gene	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_148	15718508	48 As such, it is interesting to speculate that there may be SMC-lineage specific patterning of chromatin structure that selectively controls SRF binding and subsequent recruitment of myocardin to a very select subset of SMC marker genes but not growth response genes like c- fos or skeletal and cardiac multiple CArG-containing genes.	bind
34039	2	8274	7	NULL	NULL	0	NULL	myocardin	NULL		is not recruited to	NULL				c-fos	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_148	15718508	48 As such, it is interesting to speculate that there may be SMC-lineage specific patterning of chromatin structure that selectively controls SRF binding and subsequent recruitment of myocardin to a very select subset of SMC marker genes but not growth response genes like c- fos or skeletal and cardiac multiple CArG-containing genes.	bind
34040	3	8274	7	10	NULL	0	NULL	myocardin			is not recruited to					multiple CArG-containing genes		skeletal			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_148	15718508	48 As such, it is interesting to speculate that there may be SMC-lineage specific patterning of chromatin structure that selectively controls SRF binding and subsequent recruitment of myocardin to a very select subset of SMC marker genes but not growth response genes like c- fos or skeletal and cardiac multiple CArG-containing genes.	bind
34041	4	8274	7	10	NULL	0	NULL	myocardin			is not recruited to					multiple CArG-containing genes		cardiac			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_148	15718508	48 As such, it is interesting to speculate that there may be SMC-lineage specific patterning of chromatin structure that selectively controls SRF binding and subsequent recruitment of myocardin to a very select subset of SMC marker genes but not growth response genes like c- fos or skeletal and cardiac multiple CArG-containing genes.	bind
34059	5	8274	7	10	NULL	0	NULL	statement 10			controls		may;;selectively			statement 1					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_148	15718508	48 As such, it is interesting to speculate that there may be SMC-lineage specific patterning of chromatin structure that selectively controls SRF binding and subsequent recruitment of myocardin to a very select subset of SMC marker genes but not growth response genes like c- fos or skeletal and cardiac multiple CArG-containing genes.	bind
34060	6	8274	7	10	NULL	0	NULL	statement 10			controls		may;;selectively			statement 2					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_148	15718508	48 As such, it is interesting to speculate that there may be SMC-lineage specific patterning of chromatin structure that selectively controls SRF binding and subsequent recruitment of myocardin to a very select subset of SMC marker genes but not growth response genes like c- fos or skeletal and cardiac multiple CArG-containing genes.	bind
34061	7	8274	7	10	NULL	0	NULL	statement 10			controls		may;;selectively			statement 3					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_148	15718508	48 As such, it is interesting to speculate that there may be SMC-lineage specific patterning of chromatin structure that selectively controls SRF binding and subsequent recruitment of myocardin to a very select subset of SMC marker genes but not growth response genes like c- fos or skeletal and cardiac multiple CArG-containing genes.	bind
34062	8	8274	7	10	NULL	0	NULL	statement 10			controls		may;;selectively			statement 4					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_148	15718508	48 As such, it is interesting to speculate that there may be SMC-lineage specific patterning of chromatin structure that selectively controls SRF binding and subsequent recruitment of myocardin to a very select subset of SMC marker genes but not growth response genes like c- fos or skeletal and cardiac multiple CArG-containing genes.	bind
34063	9	8274	7	NULL	NULL	0	NULL	c- fos	NULL		is a type of	NULL				growth response genes	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_148	15718508	48 As such, it is interesting to speculate that there may be SMC-lineage specific patterning of chromatin structure that selectively controls SRF binding and subsequent recruitment of myocardin to a very select subset of SMC marker genes but not growth response genes like c- fos or skeletal and cardiac multiple CArG-containing genes.	bind
47533	11	8274	7	10	NULL	0	NULL	statement 10			controls		selectively			SRF		binding of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_148	15718508	48 As such, it is interesting to speculate that there may be SMC-lineage specific patterning of chromatin structure that selectively controls SRF binding and subsequent recruitment of myocardin to a very select subset of SMC marker genes but not growth response genes like c- fos or skeletal and cardiac multiple CArG-containing genes.	bind
56110	10	8274	7	10	NULL	0	NULL	chromatin		patterning of;;structure of	specific to					SMC-lineage					NULL		0	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_148	15718508	48 As such, it is interesting to speculate that there may be SMC-lineage specific patterning of chromatin structure that selectively controls SRF binding and subsequent recruitment of myocardin to a very select subset of SMC marker genes but not growth response genes like c- fos or skeletal and cardiac multiple CArG-containing genes.	bind
27577	1	8275	6	13	NULL	NULL	NULL	SRF	GP		bind					SM alpha-actin	GP			CArG element of promoter	NULL	A404 SMC progenitor line	NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_147	15718508	48 Briefly, we found selective enrichment of SRF binding to CArG-containing regions of SMC promoters, including the  SM alpha-actin and  SM-MHC genes, within intact chromatin after retinoic acid - induced expression of SMC marker genes in an A404 SMC progenitor line developed in our laboratory.	bind
27578	2	8275	6	13	NULL	NULL	NULL	SRF	GP		bind					SM-MHC gene	GP			CArG element of promoter	NULL	A404 SMC progenitor line	NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_147	15718508	48 Briefly, we found selective enrichment of SRF binding to CArG-containing regions of SMC promoters, including the  SM alpha-actin and  SM-MHC genes, within intact chromatin after retinoic acid - induced expression of SMC marker genes in an A404 SMC progenitor line developed in our laboratory.	bind
27580	3	8275	6	13	NULL	NULL	NULL	retinoic acid	Chemical		induces					SMC marker gene	GP	expression of			NULL	A404 SMC progenitor line	NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_147	15718508	48 Briefly, we found selective enrichment of SRF binding to CArG-containing regions of SMC promoters, including the  SM alpha-actin and  SM-MHC genes, within intact chromatin after retinoic acid - induced expression of SMC marker genes in an A404 SMC progenitor line developed in our laboratory.	bind
27582	4	8275	6	13	NULL	NULL	NULL	statement 1	Process		occurs after					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_147	15718508	48 Briefly, we found selective enrichment of SRF binding to CArG-containing regions of SMC promoters, including the  SM alpha-actin and  SM-MHC genes, within intact chromatin after retinoic acid - induced expression of SMC marker genes in an A404 SMC progenitor line developed in our laboratory.	bind
27583	5	8275	6	13	NULL	NULL	NULL	statement 2	Process		occurs after					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_147	15718508	48 Briefly, we found selective enrichment of SRF binding to CArG-containing regions of SMC promoters, including the  SM alpha-actin and  SM-MHC genes, within intact chromatin after retinoic acid - induced expression of SMC marker genes in an A404 SMC progenitor line developed in our laboratory.	bind
34073	1	8275	7	NULL	NULL	0	NULL	SRF	NULL		bind	NULL				 SM alpha-actin	NULL			CArG-containing regions of promoter	NULL	A404 SMC progenitor line	NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_147	15718508	48 Briefly, we found selective enrichment of SRF binding to CArG-containing regions of SMC promoters, including the  SM alpha-actin and  SM-MHC genes, within intact chromatin after retinoic acid - induced expression of SMC marker genes in an A404 SMC progenitor line developed in our laboratory.	bind
34076	2	8275	7	NULL	NULL	0	NULL	SRF	NULL		bind	NULL				SM-MHC genes	NULL			CArG-containing regions of promoter	NULL	A404 SMC progenitor line	NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_147	15718508	48 Briefly, we found selective enrichment of SRF binding to CArG-containing regions of SMC promoters, including the  SM alpha-actin and  SM-MHC genes, within intact chromatin after retinoic acid - induced expression of SMC marker genes in an A404 SMC progenitor line developed in our laboratory.	bind
34078	3	8275	7	NULL	NULL	0	NULL	retinoic acid	NULL		induce	NULL				SMC marker gene	NULL	expression of			NULL	A404 SMC progenitor line	NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_147	15718508	48 Briefly, we found selective enrichment of SRF binding to CArG-containing regions of SMC promoters, including the  SM alpha-actin and  SM-MHC genes, within intact chromatin after retinoic acid - induced expression of SMC marker genes in an A404 SMC progenitor line developed in our laboratory.	bind
34079	4	8275	7	NULL	NULL	0	NULL	statement 1	NULL		occurs after	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_147	15718508	48 Briefly, we found selective enrichment of SRF binding to CArG-containing regions of SMC promoters, including the  SM alpha-actin and  SM-MHC genes, within intact chromatin after retinoic acid - induced expression of SMC marker genes in an A404 SMC progenitor line developed in our laboratory.	bind
34081	5	8275	7	NULL	NULL	0	NULL	statement 2	NULL		occurs after	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_147	15718508	48 Briefly, we found selective enrichment of SRF binding to CArG-containing regions of SMC promoters, including the  SM alpha-actin and  SM-MHC genes, within intact chromatin after retinoic acid - induced expression of SMC marker genes in an A404 SMC progenitor line developed in our laboratory.	bind
27584	1	8276	6	13	NULL	NULL	NULL	collagen	GP		bind					fibronectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_3_238_s_199	12855673	48 Thus, although the r/r mutation was designed to encode collagenase resistance, it also alters collagen binding to fibronectin.	bind
27585	2	8276	6	13	NULL	NULL	NULL	r/r mutation	Process		alters					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_3_238_s_199	12855673	48 Thus, although the r/r mutation was designed to encode collagenase resistance, it also alters collagen binding to fibronectin.	bind
27586	3	8276	6	13	NULL	NULL	NULL	r/r mutation	Process		encodes					collagenase resistance	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_3_238_s_199	12855673	48 Thus, although the r/r mutation was designed to encode collagenase resistance, it also alters collagen binding to fibronectin.	bind
34083	1	8276	7	NULL	NULL	0	NULL	collagen 	NULL		bind	NULL				fibronectin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_93_3_238_s_199	12855673	48 Thus, although the r/r mutation was designed to encode collagenase resistance, it also alters collagen binding to fibronectin.	bind
34085	2	8276	7	NULL	NULL	0	NULL	r/r mutation	NULL		encode	NULL				collagenase resistance	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_93_3_238_s_199	12855673	48 Thus, although the r/r mutation was designed to encode collagenase resistance, it also alters collagen binding to fibronectin.	bind
34087	3	8276	7	NULL	NULL	0	NULL	r/r mutation	NULL		alters	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_93_3_238_s_199	12855673	48 Thus, although the r/r mutation was designed to encode collagenase resistance, it also alters collagen binding to fibronectin.	bind
27589	1	8277	6	13	NULL	NULL	NULL	Vpr protein	GP	Human immunodeficiency virus type 1	bind					uracil DNA glycosylase	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_581_s_458	11788722	49       Bouhamdan,M., Benichou,S., Rey,F., Navarro,J.M., Agostini,I., Spire,B., Camonis,J., Slupphaug,G., Vigne,R., Benarous,R. and Sire,J. (1996) Human immunodeficiency virus type 1 Vpr protein binds to the uracil DNA glycosylase DNA repair enzyme.	bind
27590	2	8277	6	13	NULL	NULL	NULL	uracil DNA glycosylase	GP		is a type of					DNA repair enzyme	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_581_s_458	11788722	49       Bouhamdan,M., Benichou,S., Rey,F., Navarro,J.M., Agostini,I., Spire,B., Camonis,J., Slupphaug,G., Vigne,R., Benarous,R. and Sire,J. (1996) Human immunodeficiency virus type 1 Vpr protein binds to the uracil DNA glycosylase DNA repair enzyme.	bind
34092	1	8277	7	NULL	NULL	0	NULL	Vpr protein	NULL	Human immunodeficiency virus type 1	binds to	NULL				uracil DNA glycosylase DNA repair enzyme	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_581_s_458	11788722	49       Bouhamdan,M., Benichou,S., Rey,F., Navarro,J.M., Agostini,I., Spire,B., Camonis,J., Slupphaug,G., Vigne,R., Benarous,R. and Sire,J. (1996) Human immunodeficiency virus type 1 Vpr protein binds to the uracil DNA glycosylase DNA repair enzyme.	bind
46831	2	8277	7	10	NULL	0	NULL	uracil DNA glycosylase	NULL		is a type of	NULL				DNA repair enzyme	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_2_581_s_458	11788722	49       Bouhamdan,M., Benichou,S., Rey,F., Navarro,J.M., Agostini,I., Spire,B., Camonis,J., Slupphaug,G., Vigne,R., Benarous,R. and Sire,J. (1996) Human immunodeficiency virus type 1 Vpr protein binds to the uracil DNA glycosylase DNA repair enzyme.	bind
28349	1	8278	6	13	NULL	NULL	NULL	70kD protein	GP		bind		specifically			GM-CSF	GP	human		AU-rich region of 3' UTR	NULL	human embryonic lung fibroblasts	NULL	NULL	NULL	NULL	gw60_circulationres_82_7_794_s_230	9562439	49  Five distinct proteins, 70, 45, 40, 38, and 32.5 kD, which specifically bind to the AU-rich region of human GM-CSF 3' UTR, were found in human embryonic lung fibroblasts.	bind
28350	2	8278	6	13	NULL	NULL	NULL	45kD protein	GP		bind		specifically			GM-CSF	GP	human		AU-rich region of 3' UTR	NULL	human embryonic lung fibroblasts	NULL	NULL	NULL	NULL	gw60_circulationres_82_7_794_s_230	9562439	49  Five distinct proteins, 70, 45, 40, 38, and 32.5 kD, which specifically bind to the AU-rich region of human GM-CSF 3' UTR, were found in human embryonic lung fibroblasts.	bind
28351	3	8278	6	13	NULL	NULL	NULL	40 kD protein	GP		bind		specifically			GM-CSF 	GP	human		AU-rich region of 3' UTR	NULL	human embryonic lung fibroblasts	NULL	NULL	NULL	NULL	gw60_circulationres_82_7_794_s_230	9562439	49  Five distinct proteins, 70, 45, 40, 38, and 32.5 kD, which specifically bind to the AU-rich region of human GM-CSF 3' UTR, were found in human embryonic lung fibroblasts.	bind
28352	4	8278	6	13	NULL	NULL	NULL	38 kDa protein	GP		bind		specifically			GM-CSF	GP	human		AU-rich region of 3' UTR	NULL	human embryonic lung fibroblasts	NULL	NULL	NULL	NULL	gw60_circulationres_82_7_794_s_230	9562439	49  Five distinct proteins, 70, 45, 40, 38, and 32.5 kD, which specifically bind to the AU-rich region of human GM-CSF 3' UTR, were found in human embryonic lung fibroblasts.	bind
28353	5	8278	6	13	NULL	NULL	NULL	32.5 kD protein	GP		bind		specifically			GM-CSF	GP	human		AU-rich region of 3' UTR	NULL	human embryonic lung fibroblasts	NULL	NULL	NULL	NULL	gw60_circulationres_82_7_794_s_230	9562439	49  Five distinct proteins, 70, 45, 40, 38, and 32.5 kD, which specifically bind to the AU-rich region of human GM-CSF 3' UTR, were found in human embryonic lung fibroblasts.	bind
34093	1	8278	7	NULL	NULL	0	NULL	70 kD protein	NULL		binds to	NULL	specifically			GM-CSF	NULL	human		AU-rich region of 3' UTR	NULL	human embryonic lung fibroblasts	NULL	NULL	NULL	NULL	gw60_circulationres_82_7_794_s_230	9562439	49  Five distinct proteins, 70, 45, 40, 38, and 32.5 kD, which specifically bind to the AU-rich region of human GM-CSF 3' UTR, were found in human embryonic lung fibroblasts.	bind
34094	2	8278	7	NULL	NULL	0	NULL	45 kD protein	NULL		binds to	NULL	specifically			GM-CSF	NULL	human		AU-rich region of 3' UTR	NULL	human embryonic lung fibroblasts	0	NULL	NULL	NULL	gw60_circulationres_82_7_794_s_230	9562439	49  Five distinct proteins, 70, 45, 40, 38, and 32.5 kD, which specifically bind to the AU-rich region of human GM-CSF 3' UTR, were found in human embryonic lung fibroblasts.	bind
34095	3	8278	7	NULL	NULL	0	NULL	40 kD protein	NULL		binds to	NULL	specifically			GM-CSF	NULL	human		AU-rich region of 3' UTR	NULL	human embryonic lung fibroblasts	0	NULL	NULL	NULL	gw60_circulationres_82_7_794_s_230	9562439	49  Five distinct proteins, 70, 45, 40, 38, and 32.5 kD, which specifically bind to the AU-rich region of human GM-CSF 3' UTR, were found in human embryonic lung fibroblasts.	bind
34096	4	8278	7	NULL	NULL	0	NULL	38 kD protein	NULL		binds to	NULL	specifically			GM-CSF	NULL	human		AU-rich region of 3' UTR	NULL	human embryonic lung fibroblasts	0	NULL	NULL	NULL	gw60_circulationres_82_7_794_s_230	9562439	49  Five distinct proteins, 70, 45, 40, 38, and 32.5 kD, which specifically bind to the AU-rich region of human GM-CSF 3' UTR, were found in human embryonic lung fibroblasts.	bind
34097	5	8278	7	NULL	NULL	0	NULL	32.5 kD protein	NULL		binds to	NULL	specifically			GM-CSF	NULL	human		AU-rich region of 3' UTR	NULL	human embryonic lung fibroblasts	NULL	NULL	NULL	NULL	gw60_circulationres_82_7_794_s_230	9562439	49  Five distinct proteins, 70, 45, 40, 38, and 32.5 kD, which specifically bind to the AU-rich region of human GM-CSF 3' UTR, were found in human embryonic lung fibroblasts.	bind
27652	1	8279	6	13	NULL	NULL	NULL	fibroblast growth factor	GP		bind					fibroblast growth factor receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_9_2605_s_199	7586363	49  Heparan sulfate proteoglycans are obligate partners in the binding of basic fibroblast growth factors to their receptors; fibroblast growth factors do not bind to fibroblast growth factor receptors unless heparan sulfate, or its analog heparin, is present.	bind
27655	2	8279	6	13	NULL	NULL	NULL	statement 1	Process		occurs in presence of		only			heparan sulfate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_9_2605_s_199	7586363	49  Heparan sulfate proteoglycans are obligate partners in the binding of basic fibroblast growth factors to their receptors; fibroblast growth factors do not bind to fibroblast growth factor receptors unless heparan sulfate, or its analog heparin, is present.	bind
27657	3	8279	6	13	NULL	NULL	NULL	statement 1	Process		occurs in presence of		only			heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_9_2605_s_199	7586363	49  Heparan sulfate proteoglycans are obligate partners in the binding of basic fibroblast growth factors to their receptors; fibroblast growth factors do not bind to fibroblast growth factor receptors unless heparan sulfate, or its analog heparin, is present.	bind
34098	1	8279	7	10	NULL	0	NULL	fibroblast growth factors	NULL		does not bind	NULL				fibroblast growth factor receptors	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_9_2605_s_199	7586363	49  Heparan sulfate proteoglycans are obligate partners in the binding of basic fibroblast growth factors to their receptors; fibroblast growth factors do not bind to fibroblast growth factor receptors unless heparan sulfate, or its analog heparin, is present.	bind
34099	2	8279	7	NULL	NULL	0	NULL	statement 1	NULL		in absence of	NULL				heparan sulfate	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_9_2605_s_199	7586363	49  Heparan sulfate proteoglycans are obligate partners in the binding of basic fibroblast growth factors to their receptors; fibroblast growth factors do not bind to fibroblast growth factor receptors unless heparan sulfate, or its analog heparin, is present.	bind
34100	3	8279	7	NULL	NULL	0	NULL	statement 1	NULL		in absence of	NULL				heparin analog	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_9_2605_s_199	7586363	49  Heparan sulfate proteoglycans are obligate partners in the binding of basic fibroblast growth factors to their receptors; fibroblast growth factors do not bind to fibroblast growth factor receptors unless heparan sulfate, or its analog heparin, is present.	bind
34101	4	8279	7	NULL	NULL	0	NULL	fibroblast growth factors	NULL		bind	NULL				fibroblast growth factor receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_9_2605_s_199	7586363	49  Heparan sulfate proteoglycans are obligate partners in the binding of basic fibroblast growth factors to their receptors; fibroblast growth factors do not bind to fibroblast growth factor receptors unless heparan sulfate, or its analog heparin, is present.	bind
34102	5	8279	7	NULL	NULL	0	NULL	Heparan sulfate proteoglycans	NULL		are obligate partners of	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_9_2605_s_199	7586363	49  Heparan sulfate proteoglycans are obligate partners in the binding of basic fibroblast growth factors to their receptors; fibroblast growth factors do not bind to fibroblast growth factor receptors unless heparan sulfate, or its analog heparin, is present.	bind
27665	1	8280	6	13	NULL	NULL	NULL	AR	GP	intact	bind		functionaly			androgen	Chemical				NULL	hormone-dependent carcinoma	NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_79_s_451	11438457	49  Importantly, results from a past study 50  demonstrated the presence of structurally intact AR that functionally binds androgen in the majority of both hormone-dependent and -independent carcinomas.	bind
27667	2	8280	6	13	NULL	NULL	NULL	AR	GP	intact	bind		functionaly			androgen	Chemical				NULL	hormone independent carcinoma	NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_79_s_451	11438457	49  Importantly, results from a past study 50  demonstrated the presence of structurally intact AR that functionally binds androgen in the majority of both hormone-dependent and -independent carcinomas.	bind
34103	1	8280	7	10	NULL	0	NULL	AR	NULL	intact 	binds	NULL	functionally			androgen	NULL				NULL	hormone-dependent carcinomas	NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_79_s_451	11438457	49  Importantly, results from a past study 50  demonstrated the presence of structurally intact AR that functionally binds androgen in the majority of both hormone-dependent and -independent carcinomas.	bind
34104	2	8280	7	10	NULL	0	NULL	AR	NULL	intact	binds	NULL	functionally			androgen	NULL				NULL	hormone-independent carcinomas	NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_79_s_451	11438457	49  Importantly, results from a past study 50  demonstrated the presence of structurally intact AR that functionally binds androgen in the majority of both hormone-dependent and -independent carcinomas.	bind
27671	1	8281	6	13	NULL	NULL	NULL	apoA-I	GP		does not bind							mutant	W590S		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_108	12738681	49 However, an equally valid interpretation is that apoA-I fails to bind the W590S mutant in the correct orientation and therefore the appropriate conformational change of ABCA1 required to decrease calpain proteolysis does not occur.	bind
27673	2	8281	6	13	NULL	NULL	NULL	ABCA1	GP	conformational change of	decrease					calpain	GP	proteolysis of 			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_108	12738681	49 However, an equally valid interpretation is that apoA-I fails to bind the W590S mutant in the correct orientation and therefore the appropriate conformational change of ABCA1 required to decrease calpain proteolysis does not occur.	bind
34105	1	8281	7	10	NULL	0	NULL	apoA-I 	NULL		fails to bind	NULL					NULL	mutant	W590S		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_108	12738681	49 However, an equally valid interpretation is that apoA-I fails to bind the W590S mutant in the correct orientation and therefore the appropriate conformational change of ABCA1 required to decrease calpain proteolysis does not occur.	bind
34106	2	8281	7	NULL	NULL	0	NULL	ABCA1	NULL	conformational change of 	decrease	NULL				calpain	NULL	proteolysis of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_108	12738681	49 However, an equally valid interpretation is that apoA-I fails to bind the W590S mutant in the correct orientation and therefore the appropriate conformational change of ABCA1 required to decrease calpain proteolysis does not occur.	bind
34107	3	8281	7	NULL	NULL	0	NULL	statement 2	NULL		does not occur with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1178_s_108	12738681	49 However, an equally valid interpretation is that apoA-I fails to bind the W590S mutant in the correct orientation and therefore the appropriate conformational change of ABCA1 required to decrease calpain proteolysis does not occur.	bind
27674	1	8282	6	13	NULL	NULL	NULL	ICP8	GP		bind					UL9 protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_66_0_347_s_214	9242911	4: binding of ICP8 to   the UL9 protein and distorted DNA.  5: ATP-dependent DNA unwinding that generates ICP8-coated DNA strands.	bind
27675	2	8282	6	13	NULL	NULL	NULL	ICP8	GP		bind					DNA	NucleicAcid	distorted			NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_66_0_347_s_214	9242911	4: binding of ICP8 to   the UL9 protein and distorted DNA.  5: ATP-dependent DNA unwinding that generates ICP8-coated DNA strands.	bind
27798	3	8282	6	13	NULL	NULL	NULL	DNA	NucleicAcid	unwinding of	generates					DNA strands	NucleicAcid	ICP8-coated			NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_66_0_347_s_214	9242911	4: binding of ICP8 to   the UL9 protein and distorted DNA.  5: ATP-dependent DNA unwinding that generates ICP8-coated DNA strands.	bind
27799	4	8282	6	13	NULL	NULL	NULL	statement 3	Process		is dependent on					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_66_0_347_s_214	9242911	4: binding of ICP8 to   the UL9 protein and distorted DNA.  5: ATP-dependent DNA unwinding that generates ICP8-coated DNA strands.	bind
34108	1	8282	7	NULL	NULL	0	NULL	ICP8	NULL		binds to	NULL				UL9 protein	NULL				NULL		0	NULL	NULL	NULL	gw60_annrevbiochem_66_0_347_s_214	9242911	4: binding of ICP8 to   the UL9 protein and distorted DNA.  5: ATP-dependent DNA unwinding that generates ICP8-coated DNA strands.	bind
34109	2	8282	7	10	NULL	0	NULL	ICP8	NULL		bind	NULL				DNA	NULL	distorted			NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_66_0_347_s_214	9242911	4: binding of ICP8 to   the UL9 protein and distorted DNA.  5: ATP-dependent DNA unwinding that generates ICP8-coated DNA strands.	bind
34110	3	8282	7	NULL	NULL	0	NULL	DNA	NULL	unwinding of	depends on	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw60_annrevbiochem_66_0_347_s_214	9242911	4: binding of ICP8 to   the UL9 protein and distorted DNA.  5: ATP-dependent DNA unwinding that generates ICP8-coated DNA strands.	bind
34111	4	8282	7	10	NULL	0	NULL	statement 2	NULL		generates	NULL				DNA strands	NULL	ICP8-coated			NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_66_0_347_s_214	9242911	4: binding of ICP8 to   the UL9 protein and distorted DNA.  5: ATP-dependent DNA unwinding that generates ICP8-coated DNA strands.	bind
27801	1	8285	6	13	NULL	NULL	NULL	4E-BP	GP		bind					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_20788_s_185	16720573	4E-BP Binding Suppresses eIF4E Ubiquitination and Degradation -- 4E-BP proteins bind eIF4E and negatively regulate cap-dependent translation initiation.	bind
27802	2	8285	6	13	NULL	NULL	NULL	statement 1	Process		suppresses					eIF4E	GP	ubiquitination of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_20788_s_185	16720573	4E-BP Binding Suppresses eIF4E Ubiquitination and Degradation -- 4E-BP proteins bind eIF4E and negatively regulate cap-dependent translation initiation.	bind
27803	3	8285	6	13	NULL	NULL	NULL	statement 1	Process		suppresses					eIF4E	GP	degradation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_20788_s_185	16720573	4E-BP Binding Suppresses eIF4E Ubiquitination and Degradation -- 4E-BP proteins bind eIF4E and negatively regulate cap-dependent translation initiation.	bind
27804	4	8285	6	13	NULL	NULL	NULL	translation	Process	initiation of	is dependent on					cap	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_20788_s_185	16720573	4E-BP Binding Suppresses eIF4E Ubiquitination and Degradation -- 4E-BP proteins bind eIF4E and negatively regulate cap-dependent translation initiation.	bind
27805	5	8285	6	13	NULL	NULL	NULL	statement 1	Process		regulates		negatively			statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_20788_s_185	16720573	4E-BP Binding Suppresses eIF4E Ubiquitination and Degradation -- 4E-BP proteins bind eIF4E and negatively regulate cap-dependent translation initiation.	bind
34115	1	8285	7	NULL	NULL	0	NULL	4E-BP	NULL	binding of	suppress	NULL				eIF4E	NULL	ubiquitination of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_20788_s_185	16720573	4E-BP Binding Suppresses eIF4E Ubiquitination and Degradation -- 4E-BP proteins bind eIF4E and negatively regulate cap-dependent translation initiation.	bind
34116	2	8285	7	NULL	NULL	0	NULL	4E-BP	NULL	binding of	suppress	NULL				eIF4E	NULL	degradation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_20788_s_185	16720573	4E-BP Binding Suppresses eIF4E Ubiquitination and Degradation -- 4E-BP proteins bind eIF4E and negatively regulate cap-dependent translation initiation.	bind
34117	3	8285	7	NULL	NULL	0	NULL	 4E-BP proteins	NULL		bind	NULL				eIF4E	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_20788_s_185	16720573	4E-BP Binding Suppresses eIF4E Ubiquitination and Degradation -- 4E-BP proteins bind eIF4E and negatively regulate cap-dependent translation initiation.	bind
34118	4	8285	7	NULL	NULL	0	NULL	translation	NULL	initiation of	depends on	NULL				cap	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_20788_s_185	16720573	4E-BP Binding Suppresses eIF4E Ubiquitination and Degradation -- 4E-BP proteins bind eIF4E and negatively regulate cap-dependent translation initiation.	bind
34119	5	8285	7	NULL	NULL	0	NULL	statement 3	NULL		regulate	NULL	negatively			statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_20788_s_185	16720573	4E-BP Binding Suppresses eIF4E Ubiquitination and Degradation -- 4E-BP proteins bind eIF4E and negatively regulate cap-dependent translation initiation.	bind
27806	1	8286	6	13	NULL	NULL	NULL	4E-BP	GP		bind					heIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_14_4068_s_92	10406811	4E-BP binding to heIF4E enhances cap affinity.	bind
27807	2	8286	6	13	NULL	NULL	NULL	statement 1	Process		enhances					cap	NucleicAcid	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_14_4068_s_92	10406811	4E-BP binding to heIF4E enhances cap affinity.	bind
34120	1	8286	7	NULL	NULL	0	NULL	4E-BP	NULL		bind	NULL				heIF4E	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_18_14_4068_s_92	10406811	4E-BP binding to heIF4E enhances cap affinity.	bind
34121	2	8286	7	10	NULL	0	NULL	statement 1	NULL		enhances	NULL				cap	NULL	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_14_4068_s_92	10406811	4E-BP binding to heIF4E enhances cap affinity.	bind
27808	1	8287	6	13	NULL	NULL	NULL	4E-BP	GP		bind					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_20788_s_269	16720573	4E-BP binds eIF4E under conditions of stress or reduced growth stimuli.	bind
27809	2	8287	6	13	NULL	NULL	NULL	statement 1	Process		occurs under conditions of					stress					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_20788_s_269	16720573	4E-BP binds eIF4E under conditions of stress or reduced growth stimuli.	bind
27810	3	8287	6	13	NULL	NULL	NULL	statement 1	Process		occurs under conditions of					growth stimuli	Process	reduced			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_20788_s_269	16720573	4E-BP binds eIF4E under conditions of stress or reduced growth stimuli.	bind
34122	1	8287	7	10	NULL	0	NULL	4E-BP	NULL		binds	NULL				 eIF4E	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_20788_s_269	16720573	4E-BP binds eIF4E under conditions of stress or reduced growth stimuli.	bind
34123	2	8287	7	10	NULL	0	NULL	statement 1	NULL		occurs under conditions of	NULL				stress	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_20788_s_269	16720573	4E-BP binds eIF4E under conditions of stress or reduced growth stimuli.	bind
46832	3	8287	7	10	NULL	0	NULL	statement 1	NULL		occurs under conditions of	NULL				growth stimuli	NULL	reduced			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_20788_s_269	16720573	4E-BP binds eIF4E under conditions of stress or reduced growth stimuli.	bind
27811	1	8288	6	13	NULL	NULL	NULL	4E-BP1	GP		is a synonym of					PHAS-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_24_21960_s_415	12668683	4E-BP1 (also known as PHAS-1) normally binds eIF4E, initiating  cap-dependent phosphorylation  ( ).	bind
27812	2	8288	6	13	NULL	NULL	NULL	4E-BP1	GP		bind					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_24_21960_s_415	12668683	4E-BP1 (also known as PHAS-1) normally binds eIF4E, initiating  cap-dependent phosphorylation  ( ).	bind
27813	3	8288	6	13	NULL	NULL	NULL	eIF4E	GP	phosphorylation of	is dependent on					cap	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_24_21960_s_415	12668683	4E-BP1 (also known as PHAS-1) normally binds eIF4E, initiating  cap-dependent phosphorylation  ( ).	bind
27814	4	8288	6	13	NULL	NULL	NULL	statement 2	Process		initiates					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_24_21960_s_415	12668683	4E-BP1 (also known as PHAS-1) normally binds eIF4E, initiating  cap-dependent phosphorylation  ( ).	bind
34124	1	8288	7	NULL	NULL	0	NULL	4E-BP1	NULL		binds	NULL	normally			eIF4E	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_24_21960_s_415	12668683	4E-BP1 (also known as PHAS-1) normally binds eIF4E, initiating  cap-dependent phosphorylation  ( ).	bind
34125	2	8288	7	NULL	NULL	0	NULL	phosphorylation	NULL		depends on	NULL				cap	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_24_21960_s_415	12668683	4E-BP1 (also known as PHAS-1) normally binds eIF4E, initiating  cap-dependent phosphorylation  ( ).	bind
34126	3	8288	7	NULL	NULL	0	NULL	statement 1	NULL		initiate	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_24_21960_s_415	12668683	4E-BP1 (also known as PHAS-1) normally binds eIF4E, initiating  cap-dependent phosphorylation  ( ).	bind
34127	4	8288	7	10	NULL	0	NULL	4E-BP1	NULL		is a synonym of	NULL				PHAS-1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_24_21960_s_415	12668683	4E-BP1 (also known as PHAS-1) normally binds eIF4E, initiating  cap-dependent phosphorylation  ( ).	bind
27815	1	8289	6	13	NULL	NULL	NULL	4E-BP1	GP		bind					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_15_10779_s_27	10753870	4E-BP1 and 4E-BP2 bind to eIF4E by a mechanism dependent on their phosphorylation state ( 31-33).	bind
27816	2	8289	6	13	NULL	NULL	NULL	4E-BP2	GP		bind					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_15_10779_s_27	10753870	4E-BP1 and 4E-BP2 bind to eIF4E by a mechanism dependent on their phosphorylation state ( 31-33).	bind
27817	3	8289	6	13	NULL	NULL	NULL	statement 1	Process		is dependent on					4E-BP1	GP	phosphorylation state of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_15_10779_s_27	10753870	4E-BP1 and 4E-BP2 bind to eIF4E by a mechanism dependent on their phosphorylation state ( 31-33).	bind
27818	4	8289	6	13	NULL	NULL	NULL	statement 2	Process		is dependent on					4E-BP2	GP	phosphorylation state of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_15_10779_s_27	10753870	4E-BP1 and 4E-BP2 bind to eIF4E by a mechanism dependent on their phosphorylation state ( 31-33).	bind
34128	1	8289	7	NULL	NULL	0	NULL	4E-BP1	NULL		binds to	NULL				eIF4E	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_15_10779_s_27	10753870	4E-BP1 and 4E-BP2 bind to eIF4E by a mechanism dependent on their phosphorylation state ( 31-33).	bind
34129	2	8289	7	NULL	NULL	0	NULL	4E-BP2	NULL		binds to	NULL				eIF4E 	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_15_10779_s_27	10753870	4E-BP1 and 4E-BP2 bind to eIF4E by a mechanism dependent on their phosphorylation state ( 31-33).	bind
34130	3	8289	7	NULL	NULL	0	NULL	statement 1	NULL		depends on	NULL				4E-BP1	NULL	phosphorylation state of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_15_10779_s_27	10753870	4E-BP1 and 4E-BP2 bind to eIF4E by a mechanism dependent on their phosphorylation state ( 31-33).	bind
34131	4	8289	7	NULL	NULL	0	NULL	statement 2	NULL		depends on	NULL				4E-BP2	NULL	phosphorylation state of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_15_10779_s_27	10753870	4E-BP1 and 4E-BP2 bind to eIF4E by a mechanism dependent on their phosphorylation state ( 31-33).	bind
27819	1	8290	6	13	NULL	NULL	NULL	4E-BP1	GP	underphosphorylated	bind		high affinity			eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_20_11831_s_25	8662663	4E-BP1 and 4E-BP2 binding to eIF4E is  regulated by phosphorylation: the underphosphorylated species possess a  high affinity for eIF4E, whereas the hyperphosphorylated species do not  bind to eIF4E( 9,  10) .	bind
27820	2	8290	6	13	NULL	NULL	NULL	4E-BP2	GP	underphosphorylated	bind		high affinity			eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_20_11831_s_25	8662663	4E-BP1 and 4E-BP2 binding to eIF4E is  regulated by phosphorylation: the underphosphorylated species possess a  high affinity for eIF4E, whereas the hyperphosphorylated species do not  bind to eIF4E( 9,  10) .	bind
27821	3	8290	6	13	NULL	NULL	NULL	4E-BP1	GP	hyperphosphorylated	does not bind					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_20_11831_s_25	8662663	4E-BP1 and 4E-BP2 binding to eIF4E is  regulated by phosphorylation: the underphosphorylated species possess a  high affinity for eIF4E, whereas the hyperphosphorylated species do not  bind to eIF4E( 9,  10) .	bind
27822	4	8290	6	13	NULL	NULL	NULL	4E-BP2	GP	hyperphosphorylated	does not bind					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_20_11831_s_25	8662663	4E-BP1 and 4E-BP2 binding to eIF4E is  regulated by phosphorylation: the underphosphorylated species possess a  high affinity for eIF4E, whereas the hyperphosphorylated species do not  bind to eIF4E( 9,  10) .	bind
34136	1	8290	7	10	NULL	0	NULL	4E-BP1		underphosphorylated	bind		high affinity			eIF4E					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_20_11831_s_25	8662663	4E-BP1 and 4E-BP2 binding to eIF4E is  regulated by phosphorylation: the underphosphorylated species possess a  high affinity for eIF4E, whereas the hyperphosphorylated species do not  bind to eIF4E( 9,  10) .	bind
34137	2	8290	7	10	NULL	0	NULL	4E-BP2		underphosphorylated	bind		high affinity			eIF4E					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_20_11831_s_25	8662663	4E-BP1 and 4E-BP2 binding to eIF4E is  regulated by phosphorylation: the underphosphorylated species possess a  high affinity for eIF4E, whereas the hyperphosphorylated species do not  bind to eIF4E( 9,  10) .	bind
46833	3	8290	7	10	NULL	0	NULL	4E-BP1		hyperphosphorylated	does not bind					eIF4E					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_20_11831_s_25	8662663	4E-BP1 and 4E-BP2 binding to eIF4E is  regulated by phosphorylation: the underphosphorylated species possess a  high affinity for eIF4E, whereas the hyperphosphorylated species do not  bind to eIF4E( 9,  10) .	bind
46834	4	8290	7	10	NULL	0	NULL	4E-BP2		hyperphosphorylated	does not bind					eIF4E					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_20_11831_s_25	8662663	4E-BP1 and 4E-BP2 binding to eIF4E is  regulated by phosphorylation: the underphosphorylated species possess a  high affinity for eIF4E, whereas the hyperphosphorylated species do not  bind to eIF4E( 9,  10) .	bind
27823	1	8291	6	13	NULL	NULL	NULL	eIF-4E	GP		is a type of					eukaryotic initiation factor 4E	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_2_283_s_65	9728910	4E-BP1 binds to eukaryotic initiation factor 4E (eIF-4E), the mRNA 7-methylguanylate (M7-GppN) cap-binding protein, and inhibits formation of the initiation complex.	bind
27824	2	8291	6	13	NULL	NULL	NULL	7-methylguanylate 	NucleicAcid		is					M7-GppN	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_2_283_s_65	9728910	4E-BP1 binds to eukaryotic initiation factor 4E (eIF-4E), the mRNA 7-methylguanylate (M7-GppN) cap-binding protein, and inhibits formation of the initiation complex.	bind
27825	3	8291	6	13	NULL	NULL	NULL	4E-BP1	GP		bind					eIF-4E	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_2_283_s_65	9728910	4E-BP1 binds to eukaryotic initiation factor 4E (eIF-4E), the mRNA 7-methylguanylate (M7-GppN) cap-binding protein, and inhibits formation of the initiation complex.	bind
27826	4	8291	6	13	NULL	NULL	NULL	4E-BP1	GP		bind					M7-GppN cap binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_2_283_s_65	9728910	4E-BP1 binds to eukaryotic initiation factor 4E (eIF-4E), the mRNA 7-methylguanylate (M7-GppN) cap-binding protein, and inhibits formation of the initiation complex.	bind
27827	5	8291	6	13	NULL	NULL	NULL	statement 3	Process		inhibits					initiation complex	GP	formation of			NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_2_283_s_65	9728910	4E-BP1 binds to eukaryotic initiation factor 4E (eIF-4E), the mRNA 7-methylguanylate (M7-GppN) cap-binding protein, and inhibits formation of the initiation complex.	bind
27828	6	8291	6	13	NULL	NULL	NULL	statement 4	Process		inhibits					initiation complex	GP	formation of			NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_2_283_s_65	9728910	4E-BP1 binds to eukaryotic initiation factor 4E (eIF-4E), the mRNA 7-methylguanylate (M7-GppN) cap-binding protein, and inhibits formation of the initiation complex.	bind
34138	1	8291	7	NULL	NULL	0	NULL	4E-BP1	NULL		binds to	NULL				eIF-4E	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_21_2_283_s_65	9728910	4E-BP1 binds to eukaryotic initiation factor 4E (eIF-4E), the mRNA 7-methylguanylate (M7-GppN) cap-binding protein, and inhibits formation of the initiation complex.	bind
34139	2	8291	7	NULL	NULL	0	NULL	4E-BP1	NULL		binds to	NULL				M7-GppN cap-binding protein	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_21_2_283_s_65	9728910	4E-BP1 binds to eukaryotic initiation factor 4E (eIF-4E), the mRNA 7-methylguanylate (M7-GppN) cap-binding protein, and inhibits formation of the initiation complex.	bind
34140	3	8291	7	NULL	NULL	0	NULL	statement 1	NULL		inhibits	NULL				initiation complex	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_neuron_21_2_283_s_65	9728910	4E-BP1 binds to eukaryotic initiation factor 4E (eIF-4E), the mRNA 7-methylguanylate (M7-GppN) cap-binding protein, and inhibits formation of the initiation complex.	bind
34141	4	8291	7	NULL	NULL	0	NULL	statement 2	NULL		inhibits	NULL				initiation complex	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_neuron_21_2_283_s_65	9728910	4E-BP1 binds to eukaryotic initiation factor 4E (eIF-4E), the mRNA 7-methylguanylate (M7-GppN) cap-binding protein, and inhibits formation of the initiation complex.	bind
34142	5	8291	7	10	NULL	0	NULL	eIF-4E	NULL		is a type of	NULL				eukaryotic initiation factor 4E	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_2_283_s_65	9728910	4E-BP1 binds to eukaryotic initiation factor 4E (eIF-4E), the mRNA 7-methylguanylate (M7-GppN) cap-binding protein, and inhibits formation of the initiation complex.	bind
34143	6	8291	7	NULL	NULL	0	NULL	M7-GppN	NULL		is	NULL				mRNA 7-methylguanylate	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_21_2_283_s_65	9728910	4E-BP1 binds to eukaryotic initiation factor 4E (eIF-4E), the mRNA 7-methylguanylate (M7-GppN) cap-binding protein, and inhibits formation of the initiation complex.	bind
27829	1	8292	6	13	NULL	NULL	NULL	protein translation	Process		is dependent on					cap	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_23_6_2333_s_101	12657692	4E-BP1 normally binds to eIF4E, thereby inhibiting cap-dependent protein translation (Gingras et al., 1999  ).	bind
27830	2	8292	6	13	NULL	NULL	NULL	4E-BP1	GP		bind					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_23_6_2333_s_101	12657692	4E-BP1 normally binds to eIF4E, thereby inhibiting cap-dependent protein translation (Gingras et al., 1999  ).	bind
27831	3	8292	6	13	NULL	NULL	NULL	statement 2	Process		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_23_6_2333_s_101	12657692	4E-BP1 normally binds to eIF4E, thereby inhibiting cap-dependent protein translation (Gingras et al., 1999  ).	bind
34144	1	8292	7	NULL	NULL	0	NULL	4E-BP1	NULL		binds	NULL	normally			eIF4E	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_23_6_2333_s_101	12657692	4E-BP1 normally binds to eIF4E, thereby inhibiting cap-dependent protein translation (Gingras et al., 1999  ).	bind
34145	2	8292	7	NULL	NULL	0	NULL	protein translation	NULL		depends on	NULL				cap	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_23_6_2333_s_101	12657692	4E-BP1 normally binds to eIF4E, thereby inhibiting cap-dependent protein translation (Gingras et al., 1999  ).	bind
34146	3	8292	7	NULL	NULL	0	NULL	statement 1	NULL		inhibits	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_23_6_2333_s_101	12657692	4E-BP1 normally binds to eIF4E, thereby inhibiting cap-dependent protein translation (Gingras et al., 1999  ).	bind
27832	1	8293	6	13	NULL	NULL	NULL	eIF4E	GP	phosphorylated	bind					capped mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_5_3303_s_207	11723111	4E-BP1 Stabilizes the Binding of Phosphorylated eIF4E to Capped mRNA-- Since eIF4E interacts with other proteins  in vivo (eIF4G, 4E-BPs), it was important to examine whether they modified the effect of phosphorylation on the binding of eIF4E to capped RNA.	bind
27833	2	8293	6	13	NULL	NULL	NULL	4E-BP1	GP		stabilizes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_5_3303_s_207	11723111	4E-BP1 Stabilizes the Binding of Phosphorylated eIF4E to Capped mRNA-- Since eIF4E interacts with other proteins  in vivo (eIF4G, 4E-BPs), it was important to examine whether they modified the effect of phosphorylation on the binding of eIF4E to capped RNA.	bind
27834	3	8293	6	13	NULL	NULL	NULL	eIF4E 	GP		interacts with					eIF4G	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_5_3303_s_207	11723111	4E-BP1 Stabilizes the Binding of Phosphorylated eIF4E to Capped mRNA-- Since eIF4E interacts with other proteins  in vivo (eIF4G, 4E-BPs), it was important to examine whether they modified the effect of phosphorylation on the binding of eIF4E to capped RNA.	bind
27835	4	8293	6	13	NULL	NULL	NULL	eIF4E	GP		interacts with					4E-BPs	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_5_3303_s_207	11723111	4E-BP1 Stabilizes the Binding of Phosphorylated eIF4E to Capped mRNA-- Since eIF4E interacts with other proteins  in vivo (eIF4G, 4E-BPs), it was important to examine whether they modified the effect of phosphorylation on the binding of eIF4E to capped RNA.	bind
27836	5	8293	6	13	NULL	NULL	NULL	eIF4E	GP		bind					capped RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_5_3303_s_207	11723111	4E-BP1 Stabilizes the Binding of Phosphorylated eIF4E to Capped mRNA-- Since eIF4E interacts with other proteins  in vivo (eIF4G, 4E-BPs), it was important to examine whether they modified the effect of phosphorylation on the binding of eIF4E to capped RNA.	bind
34147	1	8293	7	NULL	NULL	0	NULL	eIF4E	NULL	phosphorylated	binds	NULL				Capped mRNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_5_3303_s_207	11723111	4E-BP1 Stabilizes the Binding of Phosphorylated eIF4E to Capped mRNA-- Since eIF4E interacts with other proteins  in vivo (eIF4G, 4E-BPs), it was important to examine whether they modified the effect of phosphorylation on the binding of eIF4E to capped RNA.	bind
34148	2	8293	7	NULL	NULL	0	NULL	4E-BP1	NULL		stabilizes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_5_3303_s_207	11723111	4E-BP1 Stabilizes the Binding of Phosphorylated eIF4E to Capped mRNA-- Since eIF4E interacts with other proteins  in vivo (eIF4G, 4E-BPs), it was important to examine whether they modified the effect of phosphorylation on the binding of eIF4E to capped RNA.	bind
34149	3	8293	7	NULL	NULL	0	NULL	eIF4E	NULL		interacts with	NULL				eIF4G	NULL				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_5_3303_s_207	11723111	4E-BP1 Stabilizes the Binding of Phosphorylated eIF4E to Capped mRNA-- Since eIF4E interacts with other proteins  in vivo (eIF4G, 4E-BPs), it was important to examine whether they modified the effect of phosphorylation on the binding of eIF4E to capped RNA.	bind
34150	4	8293	7	NULL	NULL	0	NULL	eIF4E	NULL		interacts with	NULL				4E-BPs	NULL				NULL	in vivo	0	NULL	NULL	NULL	gw60_jbiolchem_277_5_3303_s_207	11723111	4E-BP1 Stabilizes the Binding of Phosphorylated eIF4E to Capped mRNA-- Since eIF4E interacts with other proteins  in vivo (eIF4G, 4E-BPs), it was important to examine whether they modified the effect of phosphorylation on the binding of eIF4E to capped RNA.	bind
27837	1	8294	6	13	NULL	NULL	NULL	4E-BP3	GP		bind					eIF4E	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_22_14002_s_8	9593750	4E-BP3 is a heat stable protein that binds to eIF4E  in vitro as well as  in vivo.	bind
27838	2	8294	6	13	NULL	NULL	NULL	4E-BP3	GP		bind					eIF4E	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_22_14002_s_8	9593750	4E-BP3 is a heat stable protein that binds to eIF4E  in vitro as well as  in vivo.	bind
27839	3	8294	6	13	NULL	NULL	NULL	4E-BP3	GP		is a type of					heat stable protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_22_14002_s_8	9593750	4E-BP3 is a heat stable protein that binds to eIF4E  in vitro as well as  in vivo.	bind
34151	1	8294	7	NULL	NULL	0	NULL	4E-BP3	NULL		binds to	NULL				eIF4E	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_273_22_14002_s_8	9593750	4E-BP3 is a heat stable protein that binds to eIF4E  in vitro as well as  in vivo.	bind
34152	2	8294	7	NULL	NULL	0	NULL	4E-BP3	NULL		binds to	NULL				eIF4E	NULL				NULL	in vivo	0	NULL	NULL	NULL	gw60_jbiolchem_273_22_14002_s_8	9593750	4E-BP3 is a heat stable protein that binds to eIF4E  in vitro as well as  in vivo.	bind
34153	3	8294	7	NULL	NULL	0	NULL	4E-BP3 	NULL		is a type of	NULL				heat stable protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_22_14002_s_8	9593750	4E-BP3 is a heat stable protein that binds to eIF4E  in vitro as well as  in vivo.	bind
27840	1	8295	6	13	NULL	NULL	NULL	4E-T	GP		bind					eIF4E	GP		dorsal site		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_16_5692_s_358	12897141	4E-T binds to the dorsal site of eIF4E ( ), a region also involved in binding eIF4G and 4E-BP1.	bind
27841	2	8295	6	13	NULL	NULL	NULL	eIF4G	GP		bind					eIF4E	GP		dorsal site 		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_16_5692_s_358	12897141	4E-T binds to the dorsal site of eIF4E ( ), a region also involved in binding eIF4G and 4E-BP1.	bind
47519	3	8295	6	13	NULL	NULL	NULL	4E-BP1	GP		bind					eIF4E	GP		dorsal site 		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_16_5692_s_358	12897141	4E-T binds to the dorsal site of eIF4E ( ), a region also involved in binding eIF4G and 4E-BP1.	bind
34154	1	8295	7	NULL	NULL	0	NULL	4E-T	NULL		binds to	NULL				eIF4E	NULL		dorsal site of		NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_16_5692_s_358	12897141	4E-T binds to the dorsal site of eIF4E ( ), a region also involved in binding eIF4G and 4E-BP1.	bind
34155	2	8295	7	NULL	NULL	0	NULL	eIF4G	NULL		binds to	NULL				eIF4E	NULL		dorsal site of		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_16_5692_s_358	12897141	4E-T binds to the dorsal site of eIF4E ( ), a region also involved in binding eIF4G and 4E-BP1.	bind
34156	3	8295	7	NULL	NULL	0	NULL	4E-BP1	NULL		binds to	NULL				eIF4E	NULL		dorsal site of		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_16_5692_s_358	12897141	4E-T binds to the dorsal site of eIF4E ( ), a region also involved in binding eIF4G and 4E-BP1.	bind
27842	1	8297	6	13	NULL	NULL	NULL	eIF4E	GP		bind					eIF4G	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24293_s_14	16798736	4EBP1 binds eIF4E, the mRNA cap-binding protein, and it represses cap-dependent translation by competitively blocking the binding of eIF4G to eIF4E ( ,  ).	bind
27843	2	8297	6	13	NULL	NULL	NULL	4EBP1	GP		bind					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24293_s_14	16798736	4EBP1 binds eIF4E, the mRNA cap-binding protein, and it represses cap-dependent translation by competitively blocking the binding of eIF4G to eIF4E ( ,  ).	bind
27844	3	8297	6	13	NULL	NULL	NULL	4EBP1	GP		bind					mRNA cap-binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24293_s_14	16798736	4EBP1 binds eIF4E, the mRNA cap-binding protein, and it represses cap-dependent translation by competitively blocking the binding of eIF4G to eIF4E ( ,  ).	bind
27845	4	8297	6	13	NULL	NULL	NULL	translation	Process		is dependent on					cap	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24293_s_14	16798736	4EBP1 binds eIF4E, the mRNA cap-binding protein, and it represses cap-dependent translation by competitively blocking the binding of eIF4G to eIF4E ( ,  ).	bind
27846	5	8297	6	13	NULL	NULL	NULL	4EBP1	GP		represses					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24293_s_14	16798736	4EBP1 binds eIF4E, the mRNA cap-binding protein, and it represses cap-dependent translation by competitively blocking the binding of eIF4G to eIF4E ( ,  ).	bind
27847	6	8297	6	13	NULL	NULL	NULL	4EBP1	GP		blocks		competitively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24293_s_14	16798736	4EBP1 binds eIF4E, the mRNA cap-binding protein, and it represses cap-dependent translation by competitively blocking the binding of eIF4G to eIF4E ( ,  ).	bind
27848	7	8297	6	13	NULL	NULL	NULL	statement 5	Process		occurs via					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24293_s_14	16798736	4EBP1 binds eIF4E, the mRNA cap-binding protein, and it represses cap-dependent translation by competitively blocking the binding of eIF4G to eIF4E ( ,  ).	bind
34177	1	8297	7	NULL	NULL	0	NULL	4EBP1	NULL		binds	NULL				eIF4E	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_34_24293_s_14	16798736	4EBP1 binds eIF4E, the mRNA cap-binding protein, and it represses cap-dependent translation by competitively blocking the binding of eIF4G to eIF4E ( ,  ).	bind
34179	2	8297	7	NULL	NULL	0	NULL	4EBP1	NULL		binds	NULL				mRNA cap-binding protein	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_34_24293_s_14	16798736	4EBP1 binds eIF4E, the mRNA cap-binding protein, and it represses cap-dependent translation by competitively blocking the binding of eIF4G to eIF4E ( ,  ).	bind
34181	3	8297	7	NULL	NULL	0	NULL	 eIF4G	NULL		bind	NULL				eIF4E	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_34_24293_s_14	16798736	4EBP1 binds eIF4E, the mRNA cap-binding protein, and it represses cap-dependent translation by competitively blocking the binding of eIF4G to eIF4E ( ,  ).	bind
34182	4	8297	7	10	NULL	0	NULL	4EBP1	NULL		repress	NULL				statement 6	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24293_s_14	16798736	4EBP1 binds eIF4E, the mRNA cap-binding protein, and it represses cap-dependent translation by competitively blocking the binding of eIF4G to eIF4E ( ,  ).	bind
34183	5	8297	7	10	NULL	0	NULL	4EBP1	NULL		blocks	NULL	competitively			statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24293_s_14	16798736	4EBP1 binds eIF4E, the mRNA cap-binding protein, and it represses cap-dependent translation by competitively blocking the binding of eIF4G to eIF4E ( ,  ).	bind
46835	6	8297	7	10	NULL	0	NULL	translation	NULL		is dependent on	NULL				cap	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_34_24293_s_14	16798736	4EBP1 binds eIF4E, the mRNA cap-binding protein, and it represses cap-dependent translation by competitively blocking the binding of eIF4G to eIF4E ( ,  ).	bind
46836	7	8297	7	10	NULL	0	NULL	statement 4	NULL		occurs via	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_34_24293_s_14	16798736	4EBP1 binds eIF4E, the mRNA cap-binding protein, and it represses cap-dependent translation by competitively blocking the binding of eIF4G to eIF4E ( ,  ).	bind
27849	1	8298	6	13	NULL	NULL	NULL	eIF-4E	GP		is a type of					7-methyl-guanosine mRNA cap binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_110_2_177_s_19	12150926	4EBP1 binds to the eIF-4E (a 7-methyl-guanosine mRNA cap binding protein) and prevents eIF-4E from binding to a scaffold protein eIF-4G, thereby inhibiting the formation of the active translational complex, eIF-4F (Sonenberg, 1996   ).	bind
27850	2	8298	6	13	NULL	NULL	NULL	4EBP1	GP		bind					eIF-4E	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_110_2_177_s_19	12150926	4EBP1 binds to the eIF-4E (a 7-methyl-guanosine mRNA cap binding protein) and prevents eIF-4E from binding to a scaffold protein eIF-4G, thereby inhibiting the formation of the active translational complex, eIF-4F (Sonenberg, 1996   ).	bind
27851	3	8298	6	13	NULL	NULL	NULL	eIF-4G	GP		is a type of					scaffold protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_110_2_177_s_19	12150926	4EBP1 binds to the eIF-4E (a 7-methyl-guanosine mRNA cap binding protein) and prevents eIF-4E from binding to a scaffold protein eIF-4G, thereby inhibiting the formation of the active translational complex, eIF-4F (Sonenberg, 1996   ).	bind
28354	4	8298	6	13	NULL	NULL	NULL	eIF-4E	GP		bind					eIF-4G	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_110_2_177_s_19	12150926	4EBP1 binds to the eIF-4E (a 7-methyl-guanosine mRNA cap binding protein) and prevents eIF-4E from binding to a scaffold protein eIF-4G, thereby inhibiting the formation of the active translational complex, eIF-4F (Sonenberg, 1996   ).	bind
28355	5	8298	6	13	NULL	NULL	NULL	statement 2	Process		prevents					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_110_2_177_s_19	12150926	4EBP1 binds to the eIF-4E (a 7-methyl-guanosine mRNA cap binding protein) and prevents eIF-4E from binding to a scaffold protein eIF-4G, thereby inhibiting the formation of the active translational complex, eIF-4F (Sonenberg, 1996   ).	bind
28357	6	8298	6	13	NULL	NULL	NULL	statement 5	Process		inhibits					active translational complex	GP	formation of 			NULL		NULL	NULL	NULL	NULL	gw60_cell_110_2_177_s_19	12150926	4EBP1 binds to the eIF-4E (a 7-methyl-guanosine mRNA cap binding protein) and prevents eIF-4E from binding to a scaffold protein eIF-4G, thereby inhibiting the formation of the active translational complex, eIF-4F (Sonenberg, 1996   ).	bind
46837	7	8298	6	13	NULL	NULL	NULL	active translational complex	GP		is					eIF-4F	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_110_2_177_s_19	12150926	4EBP1 binds to the eIF-4E (a 7-methyl-guanosine mRNA cap binding protein) and prevents eIF-4E from binding to a scaffold protein eIF-4G, thereby inhibiting the formation of the active translational complex, eIF-4F (Sonenberg, 1996   ).	bind
34185	1	8298	7	NULL	NULL	0	NULL	4EBP1	NULL		binds to	NULL				eIF-4E	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_110_2_177_s_19	12150926	4EBP1 binds to the eIF-4E (a 7-methyl-guanosine mRNA cap binding protein) and prevents eIF-4E from binding to a scaffold protein eIF-4G, thereby inhibiting the formation of the active translational complex, eIF-4F (Sonenberg, 1996   ).	bind
34187	2	8298	7	NULL	NULL	0	NULL	eIF-4E	NULL		bind	NULL				eIF-4G	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_110_2_177_s_19	12150926	4EBP1 binds to the eIF-4E (a 7-methyl-guanosine mRNA cap binding protein) and prevents eIF-4E from binding to a scaffold protein eIF-4G, thereby inhibiting the formation of the active translational complex, eIF-4F (Sonenberg, 1996   ).	bind
34188	3	8298	7	NULL	NULL	0	NULL	statement 1	NULL		prevents	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_110_2_177_s_19	12150926	4EBP1 binds to the eIF-4E (a 7-methyl-guanosine mRNA cap binding protein) and prevents eIF-4E from binding to a scaffold protein eIF-4G, thereby inhibiting the formation of the active translational complex, eIF-4F (Sonenberg, 1996   ).	bind
34189	4	8298	7	10	NULL	0	NULL	eIF-4E	NULL		is a type of	NULL				7-methyl-guanosine mRNA cap binding protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cell_110_2_177_s_19	12150926	4EBP1 binds to the eIF-4E (a 7-methyl-guanosine mRNA cap binding protein) and prevents eIF-4E from binding to a scaffold protein eIF-4G, thereby inhibiting the formation of the active translational complex, eIF-4F (Sonenberg, 1996   ).	bind
34190	5	8298	7	NULL	NULL	0	NULL	eIF-4G	NULL		is a type of	NULL				scaffold protein	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_110_2_177_s_19	12150926	4EBP1 binds to the eIF-4E (a 7-methyl-guanosine mRNA cap binding protein) and prevents eIF-4E from binding to a scaffold protein eIF-4G, thereby inhibiting the formation of the active translational complex, eIF-4F (Sonenberg, 1996   ).	bind
34192	6	8298	7	NULL	NULL	0	NULL	statement 3	NULL		inhibits	NULL				eIF-4F	NULL	 formation of			NULL		0	NULL	NULL	NULL	gw60_cell_110_2_177_s_19	12150926	4EBP1 binds to the eIF-4E (a 7-methyl-guanosine mRNA cap binding protein) and prevents eIF-4E from binding to a scaffold protein eIF-4G, thereby inhibiting the formation of the active translational complex, eIF-4F (Sonenberg, 1996   ).	bind
34194	7	8298	7	NULL	NULL	0	NULL	eIF-4F	NULL		is	NULL				active translational complex	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_110_2_177_s_19	12150926	4EBP1 binds to the eIF-4E (a 7-methyl-guanosine mRNA cap binding protein) and prevents eIF-4E from binding to a scaffold protein eIF-4G, thereby inhibiting the formation of the active translational complex, eIF-4F (Sonenberg, 1996   ).	bind
27867	1	8299	6	13	NULL	NULL	NULL	eIF4E	GP		bind					eIF4G	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_1871_s_29	10022874	4EBPs prevent eIF4E binding to eIF4G without altering mRNA binding to eIF4E ( 23,  44,  52).	bind
27868	2	8299	6	13	NULL	NULL	NULL	4EBPs	GP		prevents					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_1871_s_29	10022874	4EBPs prevent eIF4E binding to eIF4G without altering mRNA binding to eIF4E ( 23,  44,  52).	bind
27869	3	8299	6	13	NULL	NULL	NULL	eIF4E	GP		bind					mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_1871_s_29	10022874	4EBPs prevent eIF4E binding to eIF4G without altering mRNA binding to eIF4E ( 23,  44,  52).	bind
27870	4	8299	6	13	NULL	NULL	NULL	4EBPs	GP		does not alter					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_1871_s_29	10022874	4EBPs prevent eIF4E binding to eIF4G without altering mRNA binding to eIF4E ( 23,  44,  52).	bind
34197	1	8299	7	NULL	NULL	0	NULL	eIF4E	NULL		bind	NULL				eIF4G	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_3_1871_s_29	10022874	4EBPs prevent eIF4E binding to eIF4G without altering mRNA binding to eIF4E ( 23,  44,  52).	bind
34198	2	8299	7	NULL	NULL	0	NULL	mRNA	NULL		bind	NULL				eIF4E	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_3_1871_s_29	10022874	4EBPs prevent eIF4E binding to eIF4G without altering mRNA binding to eIF4E ( 23,  44,  52).	bind
34199	3	8299	7	NULL	NULL	0	NULL	4EBPs	NULL		prevents	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_3_1871_s_29	10022874	4EBPs prevent eIF4E binding to eIF4G without altering mRNA binding to eIF4E ( 23,  44,  52).	bind
34201	4	8299	7	NULL	NULL	0	NULL	statement 3	NULL		does not alter	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_1871_s_29	10022874	4EBPs prevent eIF4E binding to eIF4G without altering mRNA binding to eIF4E ( 23,  44,  52).	bind
27871	1	8300	6	13	NULL	NULL	NULL	4P-PDOT	Chemical		bind					MT1	GP				NULL		NULL	NULL	NULL	NULL	gw70_brainres_970_1_169_s_184	12706258	4P-PDOT is highly selective for MT2, and will bind MT1 as well.	bind
27874	2	8300	6	13	NULL	NULL	NULL	4P-PDOT	Chemical		selective for		highly			MT2	GP				NULL		NULL	NULL	NULL	NULL	gw70_brainres_970_1_169_s_184	12706258	4P-PDOT is highly selective for MT2, and will bind MT1 as well.	bind
34205	1	8300	7	NULL	NULL	0	NULL	4P-PDOT	NULL		selective for	NULL	highly			MT2	NULL				NULL		0	NULL	NULL	NULL	gw70_brainres_970_1_169_s_184	12706258	4P-PDOT is highly selective for MT2, and will bind MT1 as well.	bind
34207	2	8300	7	NULL	NULL	0	NULL	4P-PDOT	NULL		bind	NULL				MT1	NULL				NULL		0	NULL	NULL	NULL	gw70_brainres_970_1_169_s_184	12706258	4P-PDOT is highly selective for MT2, and will bind MT1 as well.	bind
28360	1	8301	6	13	NULL	NULL	NULL	4PS	GP		interacts with					PI 3 kinase	GP				NULL	IRS-1-deficient Mice	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_42_24670_s_100	7559579	4PS Is the Dominant Phosphoprotein Interacting with PI  3-Kinase in IRS-1-deficient MiceTo determine if 4PS was the  only, or at least the major, alternative substrate of the insulin  receptor which binds to PI 3-kinase, we performed sequential  immunoprecipitation with anti-4PS antibodies followed by  phosphotyrosine blotting and PI 3-kinase assays.	bind
28361	2	8301	6	13	NULL	NULL	NULL	4PS	GP		is a type of					phosphoprotein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_42_24670_s_100	7559579	4PS Is the Dominant Phosphoprotein Interacting with PI  3-Kinase in IRS-1-deficient MiceTo determine if 4PS was the  only, or at least the major, alternative substrate of the insulin  receptor which binds to PI 3-kinase, we performed sequential  immunoprecipitation with anti-4PS antibodies followed by  phosphotyrosine blotting and PI 3-kinase assays.	bind
34210	1	8301	7	NULL	NULL	0	NULL	4PS	NULL		interacts with	NULL				 PI 3-Kinase	NULL				NULL	IRS-1-deficient Mice	0	NULL	NULL	NULL	gw60_jbiolchem_270_42_24670_s_100	7559579	4PS Is the Dominant Phosphoprotein Interacting with PI  3-Kinase in IRS-1-deficient MiceTo determine if 4PS was the  only, or at least the major, alternative substrate of the insulin  receptor which binds to PI 3-kinase, we performed sequential  immunoprecipitation with anti-4PS antibodies followed by  phosphotyrosine blotting and PI 3-kinase assays.	bind
34212	2	8301	7	NULL	NULL	0	NULL	insulin receptor 	NULL		binds	NULL				PI 3-kinase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_42_24670_s_100	7559579	4PS Is the Dominant Phosphoprotein Interacting with PI  3-Kinase in IRS-1-deficient MiceTo determine if 4PS was the  only, or at least the major, alternative substrate of the insulin  receptor which binds to PI 3-kinase, we performed sequential  immunoprecipitation with anti-4PS antibodies followed by  phosphotyrosine blotting and PI 3-kinase assays.	bind
34216	3	8301	7	NULL	NULL	0	NULL	4PS	NULL		is a type of	NULL				 Dominant Phosphoprotein 	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_42_24670_s_100	7559579	4PS Is the Dominant Phosphoprotein Interacting with PI  3-Kinase in IRS-1-deficient MiceTo determine if 4PS was the  only, or at least the major, alternative substrate of the insulin  receptor which binds to PI 3-kinase, we performed sequential  immunoprecipitation with anti-4PS antibodies followed by  phosphotyrosine blotting and PI 3-kinase assays.	bind
27877	1	8302	6	13	NULL	NULL	NULL	EBNA1	GP		is					Epstein-Barr virus nuclear antigen	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_17_3520_s_270	11522821	5       Rawlins,D.R., Milman,G., Hayward,S.D. and Hayward,G.S. (1985) Sequence-specific DNA binding of the Epstein-Barr virus nuclear antigen (EBNA1) to clustered sites in the plasmid maintenance region.	bind
27878	2	8302	6	13	NULL	NULL	NULL	EBNA1	GP		bind		sequence specifically			DNA	NucleicAcid			clustered sites in the plasmid maintenance region	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_17_3520_s_270	11522821	5       Rawlins,D.R., Milman,G., Hayward,S.D. and Hayward,G.S. (1985) Sequence-specific DNA binding of the Epstein-Barr virus nuclear antigen (EBNA1) to clustered sites in the plasmid maintenance region.	bind
34219	1	8302	7	10	NULL	0	NULL	EBNA1			bind		sequence-specific			DNA				clustered sites in the plasmid maintenance region	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_17_3520_s_270	11522821	5       Rawlins,D.R., Milman,G., Hayward,S.D. and Hayward,G.S. (1985) Sequence-specific DNA binding of the Epstein-Barr virus nuclear antigen (EBNA1) to clustered sites in the plasmid maintenance region.	bind
34221	2	8302	7	NULL	NULL	0	NULL	EBNA1	NULL		is	NULL				Epstein-Barr virus nuclear antigen 	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_17_3520_s_270	11522821	5       Rawlins,D.R., Milman,G., Hayward,S.D. and Hayward,G.S. (1985) Sequence-specific DNA binding of the Epstein-Barr virus nuclear antigen (EBNA1) to clustered sites in the plasmid maintenance region.	bind
27881	1	8303	6	13	NULL	NULL	NULL	RNA I	GP		bind					RNA II	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_11_2401_s_195	11376159	5       Tomizawa,J. (1986) Control of ColE1 plasmid replication: binding of RNA I to RNA II and inhibition of primer formation.	bind
34279	1	8303	7	NULL	NULL	0	NULL	RNA I	NULL		bind	NULL				RNA II	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_11_2401_s_195	11376159	5       Tomizawa,J. (1986) Control of ColE1 plasmid replication: binding of RNA I to RNA II and inhibition of primer formation.	bind
27884	1	8304	6	13	NULL	NULL	NULL	gp43	GP		bind					gp45	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31685_s_233	9395510	5   Berdis and Benkovic ( 30), in their measurement of the "`shutdown"` of the gp44/62 ATPase, have reported that the binding of gp43 to gp45 in the polymerase holoenzyme increases linearly with the addition of increasing numbers of equivalents of gp43.	bind
27885	2	8304	6	13	NULL	NULL	NULL	statement 1	Process		increases upon		linearly			gp43	GP	addition of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31685_s_233	9395510	5   Berdis and Benkovic ( 30), in their measurement of the "`shutdown"` of the gp44/62 ATPase, have reported that the binding of gp43 to gp45 in the polymerase holoenzyme increases linearly with the addition of increasing numbers of equivalents of gp43.	bind
46838	3	8304	6	13	NULL	NULL	NULL	statement 1	Process		occurs in					polymerase holoenzyme	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31685_s_233	9395510	5   Berdis and Benkovic ( 30), in their measurement of the "`shutdown"` of the gp44/62 ATPase, have reported that the binding of gp43 to gp45 in the polymerase holoenzyme increases linearly with the addition of increasing numbers of equivalents of gp43.	bind
34280	1	8304	7	NULL	NULL	0	NULL	 gp43	NULL		bind	NULL				gp45	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_50_31685_s_233	9395510	5   Berdis and Benkovic ( 30), in their measurement of the "`shutdown"` of the gp44/62 ATPase, have reported that the binding of gp43 to gp45 in the polymerase holoenzyme increases linearly with the addition of increasing numbers of equivalents of gp43.	bind
34281	2	8304	7	NULL	NULL	0	NULL	statement 1	NULL		occurs in	NULL				 polymerase holoenzyme 	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_50_31685_s_233	9395510	5   Berdis and Benkovic ( 30), in their measurement of the "`shutdown"` of the gp44/62 ATPase, have reported that the binding of gp43 to gp45 in the polymerase holoenzyme increases linearly with the addition of increasing numbers of equivalents of gp43.	bind
34282	3	8304	7	NULL	NULL	0	NULL	gp43	NULL	increase of	increase	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_50_31685_s_233	9395510	5   Berdis and Benkovic ( 30), in their measurement of the "`shutdown"` of the gp44/62 ATPase, have reported that the binding of gp43 to gp45 in the polymerase holoenzyme increases linearly with the addition of increasing numbers of equivalents of gp43.	bind
27886	1	8305	6	13	NULL	NULL	NULL	tropomodulin	GP		bind					actin	GP				NULL	cardiomyocytes	NULL	NULL	NULL	NULL	gw60_circulationres_82_1_94_s_27	null	5  6  Inhibition of tropomodulin binding to actin by microinjection of anti-tropomodulin antibody into cardiomyocytes results in actin filament elongation.	bind
27891	2	8305	6	13	NULL	NULL	NULL	anti-tropomodulin antibody	GP		inhibits					statement 1	Process				NULL	cardiomyocytes	NULL	NULL	NULL	NULL	gw60_circulationres_82_1_94_s_27	null	5  6  Inhibition of tropomodulin binding to actin by microinjection of anti-tropomodulin antibody into cardiomyocytes results in actin filament elongation.	bind
27894	3	8305	6	13	NULL	NULL	NULL	statement 2	Process		results in					actin filament	GP	elongation of 			NULL	cardiomyocytes	NULL	NULL	NULL	NULL	gw60_circulationres_82_1_94_s_27	null	5  6  Inhibition of tropomodulin binding to actin by microinjection of anti-tropomodulin antibody into cardiomyocytes results in actin filament elongation.	bind
34283	1	8305	7	NULL	NULL	0	NULL	tropomodulin	NULL		bind	NULL				actin	NULL				NULL	cardiomyocytes	0	NULL	NULL	NULL	gw60_circulationres_82_1_94_s_27	null	5  6  Inhibition of tropomodulin binding to actin by microinjection of anti-tropomodulin antibody into cardiomyocytes results in actin filament elongation.	bind
34284	3	8305	7	10	NULL	0	NULL	statement 2	NULL		results in	NULL				actin filament	NULL	elongation of			NULL	cardiomyocytes	NULL	NULL	NULL	NULL	gw60_circulationres_82_1_94_s_27	null	5  6  Inhibition of tropomodulin binding to actin by microinjection of anti-tropomodulin antibody into cardiomyocytes results in actin filament elongation.	bind
46839	2	8305	7	10	NULL	0	NULL	anti-tropomodulin antibody	NULL		inhibit	NULL				statement 1	NULL				NULL	cardiomyocytes	NULL	NULL	NULL	NULL	gw60_circulationres_82_1_94_s_27	null	5  6  Inhibition of tropomodulin binding to actin by microinjection of anti-tropomodulin antibody into cardiomyocytes results in actin filament elongation.	bind
27896	1	8306	6	13	NULL	NULL	NULL	Rho	GP		bind					Rho kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_10_1186_s_208	10347093	5  A recent report suggests that the binding of Rho to Rho kinase correlates with its ability to produce cell transformation.	bind
27899	2	8306	6	13	NULL	NULL	NULL	Rho	GP		produce					cell transformation	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_10_1186_s_208	10347093	5  A recent report suggests that the binding of Rho to Rho kinase correlates with its ability to produce cell transformation.	bind
27901	3	8306	6	13	NULL	NULL	NULL	statement 1	Process		correlates with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_10_1186_s_208	10347093	5  A recent report suggests that the binding of Rho to Rho kinase correlates with its ability to produce cell transformation.	bind
34285	1	8306	7	NULL	NULL	0	NULL	Rho	NULL		bind	NULL				Rho kinase	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_10_1186_s_208	10347093	5  A recent report suggests that the binding of Rho to Rho kinase correlates with its ability to produce cell transformation.	bind
34286	2	8306	7	NULL	NULL	0	NULL	statement 1	NULL		produce	NULL				cell transformation	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_10_1186_s_208	10347093	5  A recent report suggests that the binding of Rho to Rho kinase correlates with its ability to produce cell transformation.	bind
56114	3	8306	7	10	NULL	0	NULL	statement 1			correlates with					statement 2					NULL		0	NULL	NULL	NULL	gw60_circulationres_84_10_1186_s_208	10347093	5  A recent report suggests that the binding of Rho to Rho kinase correlates with its ability to produce cell transformation.	bind
27902	1	8307	6	13	NULL	NULL	NULL	ANP	GP		bind		primarily			NPRA	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_8_841_s_25	10785505	5  ANP and BNP bind primarily to NPRA, which exerts its effect on the vasculature, causing vasodilation and inhibition of the proliferation of vascular smooth muscle cells.	bind
27903	2	8307	6	13	NULL	NULL	NULL	BNP	GP		bind		primarily			NPRA	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_8_841_s_25	10785505	5  ANP and BNP bind primarily to NPRA, which exerts its effect on the vasculature, causing vasodilation and inhibition of the proliferation of vascular smooth muscle cells.	bind
27906	3	8307	6	13	NULL	NULL	NULL	statement 1	Process		causes					vascular smooth muscle cells	Cell	vasodilation of 			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_8_841_s_25	10785505	5  ANP and BNP bind primarily to NPRA, which exerts its effect on the vasculature, causing vasodilation and inhibition of the proliferation of vascular smooth muscle cells.	bind
27907	4	8307	6	13	NULL	NULL	NULL	statement 2	Process		causes					vascular smooth muscle cells	Cell	vasodilation of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_8_841_s_25	10785505	5  ANP and BNP bind primarily to NPRA, which exerts its effect on the vasculature, causing vasodilation and inhibition of the proliferation of vascular smooth muscle cells.	bind
27908	5	8307	6	13	NULL	NULL	NULL	statement 1	Process		inhibits					vascular smooth muscle cells	Cell	proliferation of 			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_8_841_s_25	10785505	5  ANP and BNP bind primarily to NPRA, which exerts its effect on the vasculature, causing vasodilation and inhibition of the proliferation of vascular smooth muscle cells.	bind
27909	6	8307	6	13	NULL	NULL	NULL	statement 2	Process		inhibits					vascular smooth muscle cells	Cell	proliferation of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_8_841_s_25	10785505	5  ANP and BNP bind primarily to NPRA, which exerts its effect on the vasculature, causing vasodilation and inhibition of the proliferation of vascular smooth muscle cells.	bind
56115	7	8307	6	13	NULL	NULL	NULL	statement 1	Process		exerts effect on					vasculature	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_8_841_s_25	10785505	5  ANP and BNP bind primarily to NPRA, which exerts its effect on the vasculature, causing vasodilation and inhibition of the proliferation of vascular smooth muscle cells.	bind
56116	8	8307	6	13	NULL	NULL	NULL	statement 2	Process		exerts effect on					vasculature	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_8_841_s_25	10785505	5  ANP and BNP bind primarily to NPRA, which exerts its effect on the vasculature, causing vasodilation and inhibition of the proliferation of vascular smooth muscle cells.	bind
34293	1	8307	7	NULL	NULL	0	NULL	 ANP	NULL		bind	NULL	primarily			NPRA	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_86_8_841_s_25	10785505	5  ANP and BNP bind primarily to NPRA, which exerts its effect on the vasculature, causing vasodilation and inhibition of the proliferation of vascular smooth muscle cells.	bind
34294	2	8307	7	NULL	NULL	0	NULL	BNP	NULL		bind	NULL	primarily			NPRA	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_86_8_841_s_25	10785505	5  ANP and BNP bind primarily to NPRA, which exerts its effect on the vasculature, causing vasodilation and inhibition of the proliferation of vascular smooth muscle cells.	bind
34295	3	8307	7	NULL	NULL	0	NULL	statement 1	NULL		exerts effect on	NULL				vasculature	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_86_8_841_s_25	10785505	5  ANP and BNP bind primarily to NPRA, which exerts its effect on the vasculature, causing vasodilation and inhibition of the proliferation of vascular smooth muscle cells.	bind
34297	4	8307	7	NULL	NULL	0	NULL	statement 2	NULL		exerts effect on	NULL				vasculature	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_86_8_841_s_25	10785505	5  ANP and BNP bind primarily to NPRA, which exerts its effect on the vasculature, causing vasodilation and inhibition of the proliferation of vascular smooth muscle cells.	bind
34298	5	8307	7	10	NULL	0	NULL	statement 3	NULL		cause	NULL				vascular smooth muscle cells	NULL	vasodilation of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_8_841_s_25	10785505	5  ANP and BNP bind primarily to NPRA, which exerts its effect on the vasculature, causing vasodilation and inhibition of the proliferation of vascular smooth muscle cells.	bind
34300	6	8307	7	10	NULL	0	NULL	statement 4	NULL		cause	NULL				vascular smooth muscle cells	NULL	vasodilation of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_8_841_s_25	10785505	5  ANP and BNP bind primarily to NPRA, which exerts its effect on the vasculature, causing vasodilation and inhibition of the proliferation of vascular smooth muscle cells.	bind
34304	7	8307	7	NULL	NULL	0	NULL	statement 3	NULL		inhibits	NULL				vascular smooth muscle cells	NULL	 proliferation of 			NULL		0	NULL	NULL	NULL	gw60_circulationres_86_8_841_s_25	10785505	5  ANP and BNP bind primarily to NPRA, which exerts its effect on the vasculature, causing vasodilation and inhibition of the proliferation of vascular smooth muscle cells.	bind
34306	8	8307	7	NULL	NULL	0	NULL	statement 4	NULL		inhibits	NULL				vascular smooth muscle cells	NULL	proliferation of			NULL		0	NULL	NULL	NULL	gw60_circulationres_86_8_841_s_25	10785505	5  ANP and BNP bind primarily to NPRA, which exerts its effect on the vasculature, causing vasodilation and inhibition of the proliferation of vascular smooth muscle cells.	bind
28363	1	8309	6	13	NULL	NULL	NULL	NFT	GP		are composed of					six tau isoforms	GP				NULL	AD	NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_14	11549586	5  Further, since NFTs in AD are composed of six tau isoforms in about equal proportions, 6- 10 but in other neurodegenerative diseases abnormal accumulations of tau proteins in neurons and/or glial cells are predominantly composed of either three or four microtubule (MT) binding repeat tau isoforms, we also asked if BSB binds all or a subset of tau inclusions.	bind
47520	3	8309	6	13	NULL	NULL	NULL	tau proteins	GP		are accumulated in		abnormally			neurons	Cell				NULL	neurodegenerative diseases	NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_14	11549586	5  Further, since NFTs in AD are composed of six tau isoforms in about equal proportions, 6- 10 but in other neurodegenerative diseases abnormal accumulations of tau proteins in neurons and/or glial cells are predominantly composed of either three or four microtubule (MT) binding repeat tau isoforms, we also asked if BSB binds all or a subset of tau inclusions.	bind
47521	4	8309	6	13	NULL	NULL	NULL	tau proteins	GP		are accumulated in		abnormally			glial cells	Cell				NULL	neurodegenerative diseases	NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_14	11549586	5  Further, since NFTs in AD are composed of six tau isoforms in about equal proportions, 6- 10 but in other neurodegenerative diseases abnormal accumulations of tau proteins in neurons and/or glial cells are predominantly composed of either three or four microtubule (MT) binding repeat tau isoforms, we also asked if BSB binds all or a subset of tau inclusions.	bind
47522	5	8309	6	13	NULL	NULL	NULL	tau proteins	GP		consists of					three or four microtubule (MT) binding repeat tau isoforms	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_14	11549586	5  Further, since NFTs in AD are composed of six tau isoforms in about equal proportions, 6- 10 but in other neurodegenerative diseases abnormal accumulations of tau proteins in neurons and/or glial cells are predominantly composed of either three or four microtubule (MT) binding repeat tau isoforms, we also asked if BSB binds all or a subset of tau inclusions.	bind
47523	6	8309	6	13	NULL	NULL	NULL	statement 5	GP		are occured in					statement 3	Cell				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_14	11549586	5  Further, since NFTs in AD are composed of six tau isoforms in about equal proportions, 6- 10 but in other neurodegenerative diseases abnormal accumulations of tau proteins in neurons and/or glial cells are predominantly composed of either three or four microtubule (MT) binding repeat tau isoforms, we also asked if BSB binds all or a subset of tau inclusions.	bind
47524	7	8309	6	13	NULL	NULL	NULL	statement 5	GP		are occured in					statement 4	Cell				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_14	11549586	5  Further, since NFTs in AD are composed of six tau isoforms in about equal proportions, 6- 10 but in other neurodegenerative diseases abnormal accumulations of tau proteins in neurons and/or glial cells are predominantly composed of either three or four microtubule (MT) binding repeat tau isoforms, we also asked if BSB binds all or a subset of tau inclusions.	bind
34307	1	8309	7	NULL	NULL	0	NULL	tau proteins	NULL		accumulates in	NULL	abnormally			neurons	NULL				NULL	neurodegenerative diseases 	NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_14	11549586	5  Further, since NFTs in AD are composed of six tau isoforms in about equal proportions, 6- 10 but in other neurodegenerative diseases abnormal accumulations of tau proteins in neurons and/or glial cells are predominantly composed of either three or four microtubule (MT) binding repeat tau isoforms, we also asked if BSB binds all or a subset of tau inclusions.	bind
34308	2	8309	7	NULL	NULL	0	NULL	tau proteins	NULL		accumulates in	NULL	abnormally			glial cells	NULL				NULL	neurodegenerative diseases 	NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_14	11549586	5  Further, since NFTs in AD are composed of six tau isoforms in about equal proportions, 6- 10 but in other neurodegenerative diseases abnormal accumulations of tau proteins in neurons and/or glial cells are predominantly composed of either three or four microtubule (MT) binding repeat tau isoforms, we also asked if BSB binds all or a subset of tau inclusions.	bind
34309	3	8309	7	NULL	NULL	0	NULL	statement 1	NULL		is composed of	NULL				MT binding repeat tau isoforms	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_14	11549586	5  Further, since NFTs in AD are composed of six tau isoforms in about equal proportions, 6- 10 but in other neurodegenerative diseases abnormal accumulations of tau proteins in neurons and/or glial cells are predominantly composed of either three or four microtubule (MT) binding repeat tau isoforms, we also asked if BSB binds all or a subset of tau inclusions.	bind
34310	4	8309	7	NULL	NULL	0	NULL	MT	NULL		is	NULL				microtubule	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_14	11549586	5  Further, since NFTs in AD are composed of six tau isoforms in about equal proportions, 6- 10 but in other neurodegenerative diseases abnormal accumulations of tau proteins in neurons and/or glial cells are predominantly composed of either three or four microtubule (MT) binding repeat tau isoforms, we also asked if BSB binds all or a subset of tau inclusions.	bind
47525	4	8309	7	NULL	NULL	0	NULL	statement 2	NULL		is composed of	NULL				MT binding repeat tau isoforms	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_14	11549586	5  Further, since NFTs in AD are composed of six tau isoforms in about equal proportions, 6- 10 but in other neurodegenerative diseases abnormal accumulations of tau proteins in neurons and/or glial cells are predominantly composed of either three or four microtubule (MT) binding repeat tau isoforms, we also asked if BSB binds all or a subset of tau inclusions.	bind
47527	5	8309	7	NULL	NULL	0	NULL	NFT	NULL		is composed of	NULL				six tau isoforms	NULL				NULL	AD	NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_937_s_14	11549586	5  Further, since NFTs in AD are composed of six tau isoforms in about equal proportions, 6- 10 but in other neurodegenerative diseases abnormal accumulations of tau proteins in neurons and/or glial cells are predominantly composed of either three or four microtubule (MT) binding repeat tau isoforms, we also asked if BSB binds all or a subset of tau inclusions.	bind
27910	1	8310	6	13	NULL	NULL	NULL	skeletal S1	GP		bind			alkali light chain 1		F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_81_5_688_s_21	9351442	5  Further, we have shown that the alkali light chain 1 of skeletal S1 can bind F-actin only when the molar ratio is low.	bind
34311	1	8310	7	10	NULL	0	NULL	skeletal S1	NULL		bind	NULL		alkali light chain 1		F-actin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_81_5_688_s_21	9351442	5  Further, we have shown that the alkali light chain 1 of skeletal S1 can bind F-actin only when the molar ratio is low.	bind
27912	1	8311	6	13	NULL	NULL	NULL	Lp(a)	GP		bind		competitively			plasminogen	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_575_s_226	10669658	5  Furthermore, the current in vitro experiments that used whole plasma failed to show any effect of plasma proteins, including high fibrinogen concentrations, on the competitive binding of Lp(a) and plasminogen.	bind
34316	1	8311	7	NULL	NULL	0	NULL	Lp(a)	NULL		binds	NULL	competitively			plasminogen	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_2_575_s_226	10669658	5  Furthermore, the current in vitro experiments that used whole plasma failed to show any effect of plasma proteins, including high fibrinogen concentrations, on the competitive binding of Lp(a) and plasminogen.	bind
27913	1	8312	6	13	NULL	NULL	NULL	SMC	Cell		adhere to					ECM substrates	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_80_5_627_s_250	9130443	5  Furthermore, using an anti - beta1 integrin antibody that augments the binding affinity of beta1 integrins, Seki et al 10  and Koyama et al 28  observed enhanced adhesion of SMCs to ECM substrates but decreased SMC migration to PDGF on Matrigel.	bind
28015	2	8312	6	13	NULL	NULL	NULL	SMC	Cell		migrate to					PDGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_80_5_627_s_250	9130443	5  Furthermore, using an anti - beta1 integrin antibody that augments the binding affinity of beta1 integrins, Seki et al 10  and Koyama et al 28  observed enhanced adhesion of SMCs to ECM substrates but decreased SMC migration to PDGF on Matrigel.	bind
28016	3	8312	6	13	NULL	NULL	NULL	anti - beta1 integrin antibody	GP		augments					beta1-integrins	GP	binding affinity of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_80_5_627_s_250	9130443	5  Furthermore, using an anti - beta1 integrin antibody that augments the binding affinity of beta1 integrins, Seki et al 10  and Koyama et al 28  observed enhanced adhesion of SMCs to ECM substrates but decreased SMC migration to PDGF on Matrigel.	bind
46840	4	8312	6	13	NULL	NULL	NULL	statement 3	Process		enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_80_5_627_s_250	9130443	5  Furthermore, using an anti - beta1 integrin antibody that augments the binding affinity of beta1 integrins, Seki et al 10  and Koyama et al 28  observed enhanced adhesion of SMCs to ECM substrates but decreased SMC migration to PDGF on Matrigel.	bind
46841	5	8312	6	13	NULL	NULL	NULL	statement 3	Process		decrease					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_80_5_627_s_250	9130443	5  Furthermore, using an anti - beta1 integrin antibody that augments the binding affinity of beta1 integrins, Seki et al 10  and Koyama et al 28  observed enhanced adhesion of SMCs to ECM substrates but decreased SMC migration to PDGF on Matrigel.	bind
34317	1	8312	7	NULL	NULL	0	NULL	anti - beta1 integrin antibody 	NULL		augments	NULL				beta1 integrins	NULL	binding affinity of			NULL		0	NULL	NULL	NULL	gw60_circulationres_80_5_627_s_250	9130443	5  Furthermore, using an anti - beta1 integrin antibody that augments the binding affinity of beta1 integrins, Seki et al 10  and Koyama et al 28  observed enhanced adhesion of SMCs to ECM substrates but decreased SMC migration to PDGF on Matrigel.	bind
34318	2	8312	7	NULL	NULL	0	NULL	SMCs	NULL		adhere to	NULL				ECM substrates	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_80_5_627_s_250	9130443	5  Furthermore, using an anti - beta1 integrin antibody that augments the binding affinity of beta1 integrins, Seki et al 10  and Koyama et al 28  observed enhanced adhesion of SMCs to ECM substrates but decreased SMC migration to PDGF on Matrigel.	bind
34319	3	8312	7	NULL	NULL	0	NULL	statement 1	NULL		enhance	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_80_5_627_s_250	9130443	5  Furthermore, using an anti - beta1 integrin antibody that augments the binding affinity of beta1 integrins, Seki et al 10  and Koyama et al 28  observed enhanced adhesion of SMCs to ECM substrates but decreased SMC migration to PDGF on Matrigel.	bind
34320	4	8312	7	NULL	NULL	0	NULL	SMC	NULL		migrate to	NULL				PDGF	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_80_5_627_s_250	9130443	5  Furthermore, using an anti - beta1 integrin antibody that augments the binding affinity of beta1 integrins, Seki et al 10  and Koyama et al 28  observed enhanced adhesion of SMCs to ECM substrates but decreased SMC migration to PDGF on Matrigel.	bind
34321	5	8312	7	NULL	NULL	0	NULL	statement 1	NULL		decrease	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_80_5_627_s_250	9130443	5  Furthermore, using an anti - beta1 integrin antibody that augments the binding affinity of beta1 integrins, Seki et al 10  and Koyama et al 28  observed enhanced adhesion of SMCs to ECM substrates but decreased SMC migration to PDGF on Matrigel.	bind
28368	1	8314	6	13	NULL	NULL	NULL	calmodulin binding proteins 	GP		inhibits					NOSIII	GP	activity of 			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_82_6_686_s_18	9546377	5  Little physiological relevance was attributed to this phenomenon, and the identification of a calmodulin-binding domain in the primary structure of NOS III 6 7 8  together with the finding that calmodulin binding proteins inhibited enzyme activity 1  strengthened the hypothesis that the binding of a Ca2+/calmodulin complex is essential to activate the constitutive enzyme.	bind
28370	2	8314	6	13	NULL	NULL	NULL	Ca2+/calmodulin complex	GP	binding of	is essential for					constitutive enzyme	GP	activation of 			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_82_6_686_s_18	9546377	5  Little physiological relevance was attributed to this phenomenon, and the identification of a calmodulin-binding domain in the primary structure of NOS III 6 7 8  together with the finding that calmodulin binding proteins inhibited enzyme activity 1  strengthened the hypothesis that the binding of a Ca2+/calmodulin complex is essential to activate the constitutive enzyme.	bind
28874	3	8314	6	13	NULL	NULL	NULL	NOSIII	GP		possesses								calmodulin-binding domain		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_82_6_686_s_18	9546377	5  Little physiological relevance was attributed to this phenomenon, and the identification of a calmodulin-binding domain in the primary structure of NOS III 6 7 8  together with the finding that calmodulin binding proteins inhibited enzyme activity 1  strengthened the hypothesis that the binding of a Ca2+/calmodulin complex is essential to activate the constitutive enzyme.	bind
34325	1	8314	7	NULL	NULL	0	NULL		NULL		is present in	NULL		calmodulin-binding domain		NOS III	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_82_6_686_s_18	9546377	5  Little physiological relevance was attributed to this phenomenon, and the identification of a calmodulin-binding domain in the primary structure of NOS III 6 7 8  together with the finding that calmodulin binding proteins inhibited enzyme activity 1  strengthened the hypothesis that the binding of a Ca2+/calmodulin complex is essential to activate the constitutive enzyme.	bind
34326	2	8314	7	10	NULL	0	NULL	calmodulin binding proteins	NULL		inhibits	NULL				NOSIII	NULL	activity of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_82_6_686_s_18	9546377	5  Little physiological relevance was attributed to this phenomenon, and the identification of a calmodulin-binding domain in the primary structure of NOS III 6 7 8  together with the finding that calmodulin binding proteins inhibited enzyme activity 1  strengthened the hypothesis that the binding of a Ca2+/calmodulin complex is essential to activate the constitutive enzyme.	bind
34327	3	8314	7	NULL	NULL	0	NULL	 Ca2+/calmodulin complex	NULL	binding of	activates	NULL	essentially			constitutive enzyme	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_82_6_686_s_18	9546377	5  Little physiological relevance was attributed to this phenomenon, and the identification of a calmodulin-binding domain in the primary structure of NOS III 6 7 8  together with the finding that calmodulin binding proteins inhibited enzyme activity 1  strengthened the hypothesis that the binding of a Ca2+/calmodulin complex is essential to activate the constitutive enzyme.	bind
28018	1	8315	6	13	NULL	NULL	NULL	vWF	GP	native	bind					GPIb	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_200_s_30	9484984	5  Moreover, the GPIb-binding domain of vWF expressed in  Escherichia coli has been shown to inhibit the binding of native vWF to GPIb, 12  and unlike native vWF, this vWF domain binds to GPIb in the absence of any modulator.	bind
28019	2	8315	6	13	NULL	NULL	NULL	vWF	GP		is expressed in			GPIb-binding domain		Escherichia coli	Organism				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_200_s_30	9484984	5  Moreover, the GPIb-binding domain of vWF expressed in  Escherichia coli has been shown to inhibit the binding of native vWF to GPIb, 12  and unlike native vWF, this vWF domain binds to GPIb in the absence of any modulator.	bind
28020	3	8315	6	13	NULL	NULL	NULL	statement 2	Process		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_200_s_30	9484984	5  Moreover, the GPIb-binding domain of vWF expressed in  Escherichia coli has been shown to inhibit the binding of native vWF to GPIb, 12  and unlike native vWF, this vWF domain binds to GPIb in the absence of any modulator.	bind
28021	4	8315	6	13	NULL	NULL	NULL	vWF	GP		bind			GPIb-binding domain		GPIb	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_200_s_30	9484984	5  Moreover, the GPIb-binding domain of vWF expressed in  Escherichia coli has been shown to inhibit the binding of native vWF to GPIb, 12  and unlike native vWF, this vWF domain binds to GPIb in the absence of any modulator.	bind
28024	5	8315	6	13	NULL	NULL	NULL	statement 4	Process		occurs in absence of					modulator	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_200_s_30	9484984	5  Moreover, the GPIb-binding domain of vWF expressed in  Escherichia coli has been shown to inhibit the binding of native vWF to GPIb, 12  and unlike native vWF, this vWF domain binds to GPIb in the absence of any modulator.	bind
34328	1	8315	7	NULL	NULL	0	NULL	 vWF	NULL	native	bind	NULL				GPIb	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_200_s_30	9484984	5  Moreover, the GPIb-binding domain of vWF expressed in  Escherichia coli has been shown to inhibit the binding of native vWF to GPIb, 12  and unlike native vWF, this vWF domain binds to GPIb in the absence of any modulator.	bind
34329	2	8315	7	10	NULL	0	NULL	statement 5	NULL		inhibits	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_200_s_30	9484984	5  Moreover, the GPIb-binding domain of vWF expressed in  Escherichia coli has been shown to inhibit the binding of native vWF to GPIb, 12  and unlike native vWF, this vWF domain binds to GPIb in the absence of any modulator.	bind
34331	3	8315	7	NULL	NULL	0	NULL	vWF	NULL		binds to	NULL		GPIb-binding domain 		GPIb	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_200_s_30	9484984	5  Moreover, the GPIb-binding domain of vWF expressed in  Escherichia coli has been shown to inhibit the binding of native vWF to GPIb, 12  and unlike native vWF, this vWF domain binds to GPIb in the absence of any modulator.	bind
34332	4	8315	7	NULL	NULL	0	NULL	statement 3	NULL		in absence of	NULL				modulator	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_200_s_30	9484984	5  Moreover, the GPIb-binding domain of vWF expressed in  Escherichia coli has been shown to inhibit the binding of native vWF to GPIb, 12  and unlike native vWF, this vWF domain binds to GPIb in the absence of any modulator.	bind
46867	5	8315	7	10	NULL	0	NULL	vWF	NULL		is expressed in	NULL		GPIb-binding domain		Escherichia coli	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_200_s_30	9484984	5  Moreover, the GPIb-binding domain of vWF expressed in  Escherichia coli has been shown to inhibit the binding of native vWF to GPIb, 12  and unlike native vWF, this vWF domain binds to GPIb in the absence of any modulator.	bind
28026	1	8316	6	13	NULL	NULL	NULL	IRS-1	GP		is					insulin receptor substrate-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_7_1081_s_19	12117720	5 -  10 The N- and C-terminal SH2 domains bind to tyrosine-phosphorylated insulin receptor substrate (IRS)-1, 11 suggesting that SHP2 is involved in positive signaling pathways serving multiple hormone receptors.	bind
28027	2	8316	6	13	NULL	NULL	NULL				bind			N-terminal SH2 domain		IRS-1	GP	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_7_1081_s_19	12117720	5 -  10 The N- and C-terminal SH2 domains bind to tyrosine-phosphorylated insulin receptor substrate (IRS)-1, 11 suggesting that SHP2 is involved in positive signaling pathways serving multiple hormone receptors.	bind
28028	3	8316	6	13	NULL	NULL	NULL				bind			C-terminal SH2 domain		IRS-1	GP	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_7_1081_s_19	12117720	5 -  10 The N- and C-terminal SH2 domains bind to tyrosine-phosphorylated insulin receptor substrate (IRS)-1, 11 suggesting that SHP2 is involved in positive signaling pathways serving multiple hormone receptors.	bind
28029	4	8316	6	13	NULL	NULL	NULL	SHP2	GP		is involved in					positive signaling pathways	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_7_1081_s_19	12117720	5 -  10 The N- and C-terminal SH2 domains bind to tyrosine-phosphorylated insulin receptor substrate (IRS)-1, 11 suggesting that SHP2 is involved in positive signaling pathways serving multiple hormone receptors.	bind
34333	1	8316	7	NULL	NULL	0	NULL		NULL		binds to	NULL		N-terminal SH2 domain		IRS-1	NULL	phosphorylated	tyrosine		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_7_1081_s_19	12117720	5 -  10 The N- and C-terminal SH2 domains bind to tyrosine-phosphorylated insulin receptor substrate (IRS)-1, 11 suggesting that SHP2 is involved in positive signaling pathways serving multiple hormone receptors.	bind
34335	2	8316	7	NULL	NULL	0	NULL		NULL		binds to	NULL		C-terminal SH2 domain		IRS-1	NULL	phophorylated	tyrosine		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_7_1081_s_19	12117720	5 -  10 The N- and C-terminal SH2 domains bind to tyrosine-phosphorylated insulin receptor substrate (IRS)-1, 11 suggesting that SHP2 is involved in positive signaling pathways serving multiple hormone receptors.	bind
34336	3	8316	7	NULL	NULL	0	NULL	SHP2	NULL		is involved in	NULL				positive signaling pathways	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_7_1081_s_19	12117720	5 -  10 The N- and C-terminal SH2 domains bind to tyrosine-phosphorylated insulin receptor substrate (IRS)-1, 11 suggesting that SHP2 is involved in positive signaling pathways serving multiple hormone receptors.	bind
34337	4	8316	7	NULL	NULL	0	NULL	statement 3	NULL		serves	NULL				multiple hormone receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_7_1081_s_19	12117720	5 -  10 The N- and C-terminal SH2 domains bind to tyrosine-phosphorylated insulin receptor substrate (IRS)-1, 11 suggesting that SHP2 is involved in positive signaling pathways serving multiple hormone receptors.	bind
34338	5	8316	7	NULL	NULL	0	NULL	statement 1	NULL		suggests	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_7_1081_s_19	12117720	5 -  10 The N- and C-terminal SH2 domains bind to tyrosine-phosphorylated insulin receptor substrate (IRS)-1, 11 suggesting that SHP2 is involved in positive signaling pathways serving multiple hormone receptors.	bind
34339	6	8316	7	NULL	NULL	0	NULL	statement 2	NULL		suggests	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_7_1081_s_19	12117720	5 -  10 The N- and C-terminal SH2 domains bind to tyrosine-phosphorylated insulin receptor substrate (IRS)-1, 11 suggesting that SHP2 is involved in positive signaling pathways serving multiple hormone receptors.	bind
46868	7	8316	7	10	NULL	0	NULL	IRS-1	NULL		is	NULL				\tinsulin receptor substrate-1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_7_1081_s_19	12117720	5 -  10 The N- and C-terminal SH2 domains bind to tyrosine-phosphorylated insulin receptor substrate (IRS)-1, 11 suggesting that SHP2 is involved in positive signaling pathways serving multiple hormone receptors.	bind
28030	1	8317	6	13	NULL	NULL	NULL	125I - Ang II	GP		bind					chromatin fragments	Chromosome	solubilized;;rat liver			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_89_12_1138_s_20	11739278	5 -  7 Re and colleagues further demonstrated 125I - Ang II binding to solubilized rat liver chromatin fragments, the existence of a discrete Ang II - binding nucleoprotein particle by deoxynucleoprotein gel electrophoresis, and direct effects of nuclear angiotensin on transcription.	bind
56117	2	8317	6	13	NULL	NULL	NULL	angiotensin	GP	nuclear	effect		directly			transcription	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_89_12_1138_s_20	11739278	5 -  7 Re and colleagues further demonstrated 125I - Ang II binding to solubilized rat liver chromatin fragments, the existence of a discrete Ang II - binding nucleoprotein particle by deoxynucleoprotein gel electrophoresis, and direct effects of nuclear angiotensin on transcription.	bind
34340	1	8317	7	10	NULL	0	NULL	125I - Ang II 	NULL		bind	NULL				chromatin fragments	NULL	solubilized;;rat liver			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_89_12_1138_s_20	11739278	5 -  7 Re and colleagues further demonstrated 125I - Ang II binding to solubilized rat liver chromatin fragments, the existence of a discrete Ang II - binding nucleoprotein particle by deoxynucleoprotein gel electrophoresis, and direct effects of nuclear angiotensin on transcription.	bind
34341	2	8317	7	NULL	NULL	0	NULL	angiotensin	NULL	nuclear	effect	NULL	directly			transcription	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_89_12_1138_s_20	11739278	5 -  7 Re and colleagues further demonstrated 125I - Ang II binding to solubilized rat liver chromatin fragments, the existence of a discrete Ang II - binding nucleoprotein particle by deoxynucleoprotein gel electrophoresis, and direct effects of nuclear angiotensin on transcription.	bind
28031	1	8318	6	13	NULL	NULL	NULL	BTC	GP		bind					ErbB1/ErbB1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_30	12869389	5 - 7   BTC is known to bind and stimulate homodimers of ErbB1 and ErbB4, and heterodimers of ErbB1/ErbB2, ErbB1/ErbB3, ErbB1/ErbB4, ErbB2/ErbB3, and, ErbB2/ErbB4.	bind
28032	2	8318	6	13	NULL	NULL	NULL	BTC	GP		stimulates					ErbB1/ErbB1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_30	12869389	5 - 7   BTC is known to bind and stimulate homodimers of ErbB1 and ErbB4, and heterodimers of ErbB1/ErbB2, ErbB1/ErbB3, ErbB1/ErbB4, ErbB2/ErbB3, and, ErbB2/ErbB4.	bind
28190	3	8318	6	13	NULL	NULL	NULL	BTC	GP		bind					ErbB4/ErbB4	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_30	12869389	5 - 7   BTC is known to bind and stimulate homodimers of ErbB1 and ErbB4, and heterodimers of ErbB1/ErbB2, ErbB1/ErbB3, ErbB1/ErbB4, ErbB2/ErbB3, and, ErbB2/ErbB4.	bind
28191	4	8318	6	13	NULL	NULL	NULL	BTC	GP		stimulates					ErbB4/ErbB4	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_30	12869389	5 - 7   BTC is known to bind and stimulate homodimers of ErbB1 and ErbB4, and heterodimers of ErbB1/ErbB2, ErbB1/ErbB3, ErbB1/ErbB4, ErbB2/ErbB3, and, ErbB2/ErbB4.	bind
28192	5	8318	6	13	NULL	NULL	NULL	BTC	GP		bind					ErbB1/ErbB2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_30	12869389	5 - 7   BTC is known to bind and stimulate homodimers of ErbB1 and ErbB4, and heterodimers of ErbB1/ErbB2, ErbB1/ErbB3, ErbB1/ErbB4, ErbB2/ErbB3, and, ErbB2/ErbB4.	bind
28193	6	8318	6	13	NULL	NULL	NULL	BTC	GP		stimulates					ErbB1/ErbB2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_30	12869389	5 - 7   BTC is known to bind and stimulate homodimers of ErbB1 and ErbB4, and heterodimers of ErbB1/ErbB2, ErbB1/ErbB3, ErbB1/ErbB4, ErbB2/ErbB3, and, ErbB2/ErbB4.	bind
28194	7	8318	6	13	NULL	NULL	NULL	BTC	GP		bind					ErbB1/ErbB3	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_30	12869389	5 - 7   BTC is known to bind and stimulate homodimers of ErbB1 and ErbB4, and heterodimers of ErbB1/ErbB2, ErbB1/ErbB3, ErbB1/ErbB4, ErbB2/ErbB3, and, ErbB2/ErbB4.	bind
28195	8	8318	6	13	NULL	NULL	NULL	BTC	GP		stimulates					ErbB1/ErbB3	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_30	12869389	5 - 7   BTC is known to bind and stimulate homodimers of ErbB1 and ErbB4, and heterodimers of ErbB1/ErbB2, ErbB1/ErbB3, ErbB1/ErbB4, ErbB2/ErbB3, and, ErbB2/ErbB4.	bind
28196	9	8318	6	13	NULL	NULL	NULL	BTC	GP		bind					ErbB1/ErbB4	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_30	12869389	5 - 7   BTC is known to bind and stimulate homodimers of ErbB1 and ErbB4, and heterodimers of ErbB1/ErbB2, ErbB1/ErbB3, ErbB1/ErbB4, ErbB2/ErbB3, and, ErbB2/ErbB4.	bind
28197	10	8318	6	13	NULL	NULL	NULL	BTC	GP		stimulates					ErbB1/ErbB4	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_30	12869389	5 - 7   BTC is known to bind and stimulate homodimers of ErbB1 and ErbB4, and heterodimers of ErbB1/ErbB2, ErbB1/ErbB3, ErbB1/ErbB4, ErbB2/ErbB3, and, ErbB2/ErbB4.	bind
28198	11	8318	6	13	NULL	NULL	NULL	BTC	GP		bind					ErbB2/ErbB3	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_30	12869389	5 - 7   BTC is known to bind and stimulate homodimers of ErbB1 and ErbB4, and heterodimers of ErbB1/ErbB2, ErbB1/ErbB3, ErbB1/ErbB4, ErbB2/ErbB3, and, ErbB2/ErbB4.	bind
28199	12	8318	6	13	NULL	NULL	NULL	BTC	GP		stimulates					ErbB2/ErbB3	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_30	12869389	5 - 7   BTC is known to bind and stimulate homodimers of ErbB1 and ErbB4, and heterodimers of ErbB1/ErbB2, ErbB1/ErbB3, ErbB1/ErbB4, ErbB2/ErbB3, and, ErbB2/ErbB4.	bind
28200	13	8318	6	13	NULL	NULL	NULL	BTC	GP		bind					ErbB2/ErbB4	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_30	12869389	5 - 7   BTC is known to bind and stimulate homodimers of ErbB1 and ErbB4, and heterodimers of ErbB1/ErbB2, ErbB1/ErbB3, ErbB1/ErbB4, ErbB2/ErbB3, and, ErbB2/ErbB4.	bind
28201	14	8318	6	13	NULL	NULL	NULL	BTC	GP		stimulates					ErbB2/ErbB4	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_30	12869389	5 - 7   BTC is known to bind and stimulate homodimers of ErbB1 and ErbB4, and heterodimers of ErbB1/ErbB2, ErbB1/ErbB3, ErbB1/ErbB4, ErbB2/ErbB3, and, ErbB2/ErbB4.	bind
34344	1	8318	7	10	NULL	0	NULL	BTC	NULL		bind	NULL				ErbB1 homodimer	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_30	12869389	5 - 7   BTC is known to bind and stimulate homodimers of ErbB1 and ErbB4, and heterodimers of ErbB1/ErbB2, ErbB1/ErbB3, ErbB1/ErbB4, ErbB2/ErbB3, and, ErbB2/ErbB4.	bind
34345	2	8318	7	10	NULL	0	NULL	BTC 	NULL		bind	NULL				ErbB4 homodimer	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_30	12869389	5 - 7   BTC is known to bind and stimulate homodimers of ErbB1 and ErbB4, and heterodimers of ErbB1/ErbB2, ErbB1/ErbB3, ErbB1/ErbB4, ErbB2/ErbB3, and, ErbB2/ErbB4.	bind
34347	3	8318	7	10	NULL	0	NULL	statement 1	NULL		stimulate	NULL				ErbB1 homodimer	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_30	12869389	5 - 7   BTC is known to bind and stimulate homodimers of ErbB1 and ErbB4, and heterodimers of ErbB1/ErbB2, ErbB1/ErbB3, ErbB1/ErbB4, ErbB2/ErbB3, and, ErbB2/ErbB4.	bind
34348	4	8318	7	10	NULL	0	NULL	statement 2	NULL		stimulate	NULL				ErbB4 homodimer	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_30	12869389	5 - 7   BTC is known to bind and stimulate homodimers of ErbB1 and ErbB4, and heterodimers of ErbB1/ErbB2, ErbB1/ErbB3, ErbB1/ErbB4, ErbB2/ErbB3, and, ErbB2/ErbB4.	bind
34350	5	8318	7	NULL	NULL	0	NULL	BTC	NULL		bind	NULL				ErbB1/ErbB2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_30	12869389	5 - 7   BTC is known to bind and stimulate homodimers of ErbB1 and ErbB4, and heterodimers of ErbB1/ErbB2, ErbB1/ErbB3, ErbB1/ErbB4, ErbB2/ErbB3, and, ErbB2/ErbB4.	bind
34351	6	8318	7	NULL	NULL	0	NULL	BTC	NULL		bind	NULL				ErbB1/ErbB3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_30	12869389	5 - 7   BTC is known to bind and stimulate homodimers of ErbB1 and ErbB4, and heterodimers of ErbB1/ErbB2, ErbB1/ErbB3, ErbB1/ErbB4, ErbB2/ErbB3, and, ErbB2/ErbB4.	bind
34354	7	8318	7	NULL	NULL	0	NULL	BTC	NULL		bind	NULL				ErbB1/ErbB4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_30	12869389	5 - 7   BTC is known to bind and stimulate homodimers of ErbB1 and ErbB4, and heterodimers of ErbB1/ErbB2, ErbB1/ErbB3, ErbB1/ErbB4, ErbB2/ErbB3, and, ErbB2/ErbB4.	bind
34355	8	8318	7	NULL	NULL	0	NULL	BTC	NULL		bind	NULL				ErbB2/ErbB3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_30	12869389	5 - 7   BTC is known to bind and stimulate homodimers of ErbB1 and ErbB4, and heterodimers of ErbB1/ErbB2, ErbB1/ErbB3, ErbB1/ErbB4, ErbB2/ErbB3, and, ErbB2/ErbB4.	bind
34358	9	8318	7	NULL	NULL	0	NULL	BTC	NULL		bind	NULL				ErbB2/ErbB4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_30	12869389	5 - 7   BTC is known to bind and stimulate homodimers of ErbB1 and ErbB4, and heterodimers of ErbB1/ErbB2, ErbB1/ErbB3, ErbB1/ErbB4, ErbB2/ErbB3, and, ErbB2/ErbB4.	bind
34364	10	8318	7	NULL	NULL	0	NULL	statement 5	NULL		stimulate	NULL				ErbB1/ErbB2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_30	12869389	5 - 7   BTC is known to bind and stimulate homodimers of ErbB1 and ErbB4, and heterodimers of ErbB1/ErbB2, ErbB1/ErbB3, ErbB1/ErbB4, ErbB2/ErbB3, and, ErbB2/ErbB4.	bind
34365	11	8318	7	NULL	NULL	0	NULL	statement 6	NULL		stimulate	NULL				ErbB1/ErbB3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_30	12869389	5 - 7   BTC is known to bind and stimulate homodimers of ErbB1 and ErbB4, and heterodimers of ErbB1/ErbB2, ErbB1/ErbB3, ErbB1/ErbB4, ErbB2/ErbB3, and, ErbB2/ErbB4.	bind
34366	12	8318	7	NULL	NULL	0	NULL	statement 7	NULL		stimulate	NULL				ErbB1/ErbB4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_30	12869389	5 - 7   BTC is known to bind and stimulate homodimers of ErbB1 and ErbB4, and heterodimers of ErbB1/ErbB2, ErbB1/ErbB3, ErbB1/ErbB4, ErbB2/ErbB3, and, ErbB2/ErbB4.	bind
34367	13	8318	7	NULL	NULL	0	NULL	statement 8	NULL		stimulate	NULL				ErbB2/ErbB3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_30	12869389	5 - 7   BTC is known to bind and stimulate homodimers of ErbB1 and ErbB4, and heterodimers of ErbB1/ErbB2, ErbB1/ErbB3, ErbB1/ErbB4, ErbB2/ErbB3, and, ErbB2/ErbB4.	bind
34368	14	8318	7	NULL	NULL	0	NULL	statement 9	NULL		stimulate	NULL				ErbB2/ErbB4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_30	12869389	5 - 7   BTC is known to bind and stimulate homodimers of ErbB1 and ErbB4, and heterodimers of ErbB1/ErbB2, ErbB1/ErbB3, ErbB1/ErbB4, ErbB2/ErbB3, and, ErbB2/ErbB4.	bind
28213	1	8320	6	13	NULL	NULL	NULL	AR	GP		bind		preferentially			ErbB1 homodimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_31	12869389	5 - 8    AR is known to preferentially bind and stimulate homodimers of ErbB1.	bind
28214	2	8320	6	13	NULL	NULL	NULL	AR	GP		stimulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_31	12869389	5 - 8    AR is known to preferentially bind and stimulate homodimers of ErbB1.	bind
34391	1	8320	7	10	NULL	0	NULL	AR	NULL		bind	NULL	preferentially			ErbB1 homodimer	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_31	12869389	5 - 8    AR is known to preferentially bind and stimulate homodimers of ErbB1.	bind
34392	2	8320	7	NULL	NULL	0	NULL	AR	NULL		stimulate	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_93_4_302_s_31	12869389	5 - 8    AR is known to preferentially bind and stimulate homodimers of ErbB1.	bind
28215	1	8321	6	13	NULL	NULL	NULL	AMP	Chemical		bind					phosphorylase a	GP	liver			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27569_s_186	8910343	5 -AMP binding to liver phosphorylase  a involves a large negative delta C p.	bind
28216	2	8321	6	13	NULL	NULL	NULL	delta C p	GP	negative	plays a role in					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27569_s_186	8910343	5 -AMP binding to liver phosphorylase  a involves a large negative delta C p.	bind
34413	1	8321	7	10	NULL	0	NULL	AMP	NULL		bind	NULL				phosphorylase a	NULL	liver			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27569_s_186	8910343	5 -AMP binding to liver phosphorylase  a involves a large negative delta C p.	bind
34414	2	8321	7	10	NULL	0	NULL	statement 1			involves					delta Cp		negative			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27569_s_186	8910343	5 -AMP binding to liver phosphorylase  a involves a large negative delta C p.	bind
28217	1	8322	6	13	NULL	NULL	NULL	Fos-Jun	GP		bind					AP-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_5_940_s_191	9157959	5 21  Blocking any one of the above steps, including  Fos-Jun binding to AP-1, could downregulate the induction of TF expression.	bind
28218	2	8322	6	13	NULL	NULL	NULL	statement 1	Process	blocking of	downregulates					TF	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_5_940_s_191	9157959	5 21  Blocking any one of the above steps, including  Fos-Jun binding to AP-1, could downregulate the induction of TF expression.	bind
34415	1	8322	7	NULL	NULL	0	NULL	Fos-Jun	NULL		bind	NULL				 AP-1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_5_940_s_191	9157959	5 21  Blocking any one of the above steps, including  Fos-Jun binding to AP-1, could downregulate the induction of TF expression.	bind
34416	2	8322	7	10	NULL	0	NULL	statement 1	NULL	blocking of	downregulate	NULL				TF	NULL	expression of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_5_940_s_191	9157959	5 21  Blocking any one of the above steps, including  Fos-Jun binding to AP-1, could downregulate the induction of TF expression.	bind
28219	1	8323	6	13	NULL	NULL	NULL	SAA	GP		is					serum amyloid A	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2355_s_19	10521364	5 6  Serum amyloid A (SAA), an apolipoprotein predominantly bound to HDL, is an acute-phase reactant that indicates systemic inflammatory activity with at least the sensitivity of CRP. 7  SAA levels were also reported to be increased in coronary atherosclerosis.	bind
28220	2	8323	6	13	NULL	NULL	NULL	SAA	GP		is a type of					apolipoprotein	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2355_s_19	10521364	5 6  Serum amyloid A (SAA), an apolipoprotein predominantly bound to HDL, is an acute-phase reactant that indicates systemic inflammatory activity with at least the sensitivity of CRP. 7  SAA levels were also reported to be increased in coronary atherosclerosis.	bind
28221	3	8323	6	13	NULL	NULL	NULL	SAA	GP		bind					HDL	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2355_s_19	10521364	5 6  Serum amyloid A (SAA), an apolipoprotein predominantly bound to HDL, is an acute-phase reactant that indicates systemic inflammatory activity with at least the sensitivity of CRP. 7  SAA levels were also reported to be increased in coronary atherosclerosis.	bind
28222	4	8323	6	13	NULL	NULL	NULL	SAA	GP	levels of	are increased in					coronary atherosclerosis	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2355_s_19	10521364	5 6  Serum amyloid A (SAA), an apolipoprotein predominantly bound to HDL, is an acute-phase reactant that indicates systemic inflammatory activity with at least the sensitivity of CRP. 7  SAA levels were also reported to be increased in coronary atherosclerosis.	bind
28262	5	8323	6	13	NULL	NULL	NULL	SAA	GP		is a type of					acute phase reactant	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2355_s_19	10521364	5 6  Serum amyloid A (SAA), an apolipoprotein predominantly bound to HDL, is an acute-phase reactant that indicates systemic inflammatory activity with at least the sensitivity of CRP. 7  SAA levels were also reported to be increased in coronary atherosclerosis.	bind
56118	6	8323	6	13	NULL	NULL	NULL	statement 3	Process		indicates					systemic inflammatory activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2355_s_19	10521364	5 6  Serum amyloid A (SAA), an apolipoprotein predominantly bound to HDL, is an acute-phase reactant that indicates systemic inflammatory activity with at least the sensitivity of CRP. 7  SAA levels were also reported to be increased in coronary atherosclerosis.	bind
34417	1	8323	7	NULL	NULL	0	NULL	SAA	NULL		bind	NULL				HDL	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2355_s_19	10521364	5 6  Serum amyloid A (SAA), an apolipoprotein predominantly bound to HDL, is an acute-phase reactant that indicates systemic inflammatory activity with at least the sensitivity of CRP. 7  SAA levels were also reported to be increased in coronary atherosclerosis.	bind
34418	2	8323	7	NULL	NULL	0	NULL	SAA	NULL		is a type of	NULL				apolipoprotein	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2355_s_19	10521364	5 6  Serum amyloid A (SAA), an apolipoprotein predominantly bound to HDL, is an acute-phase reactant that indicates systemic inflammatory activity with at least the sensitivity of CRP. 7  SAA levels were also reported to be increased in coronary atherosclerosis.	bind
34419	3	8323	7	NULL	NULL	0	NULL	SAA	NULL		is a type of	NULL				acute phase reactant	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2355_s_19	10521364	5 6  Serum amyloid A (SAA), an apolipoprotein predominantly bound to HDL, is an acute-phase reactant that indicates systemic inflammatory activity with at least the sensitivity of CRP. 7  SAA levels were also reported to be increased in coronary atherosclerosis.	bind
34420	4	8323	7	NULL	NULL	0	NULL	statement 1	NULL		indicates	NULL				systemic inflammatory activity	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2355_s_19	10521364	5 6  Serum amyloid A (SAA), an apolipoprotein predominantly bound to HDL, is an acute-phase reactant that indicates systemic inflammatory activity with at least the sensitivity of CRP. 7  SAA levels were also reported to be increased in coronary atherosclerosis.	bind
34421	5	8323	7	NULL	NULL	0	NULL	statement 1	NULL		indicate	NULL				CRP	NULL	sensitivity of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2355_s_19	10521364	5 6  Serum amyloid A (SAA), an apolipoprotein predominantly bound to HDL, is an acute-phase reactant that indicates systemic inflammatory activity with at least the sensitivity of CRP. 7  SAA levels were also reported to be increased in coronary atherosclerosis.	bind
34422	6	8323	7	NULL	NULL	0	NULL	SAA	NULL	levels of	increase in	NULL				coronary atherosclerosis	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2355_s_19	10521364	5 6  Serum amyloid A (SAA), an apolipoprotein predominantly bound to HDL, is an acute-phase reactant that indicates systemic inflammatory activity with at least the sensitivity of CRP. 7  SAA levels were also reported to be increased in coronary atherosclerosis.	bind
34423	7	8323	7	NULL	NULL	0	NULL	SAA	NULL		is	NULL				Serum amyloid A	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2355_s_19	10521364	5 6  Serum amyloid A (SAA), an apolipoprotein predominantly bound to HDL, is an acute-phase reactant that indicates systemic inflammatory activity with at least the sensitivity of CRP. 7  SAA levels were also reported to be increased in coronary atherosclerosis.	bind
28263	1	8324	6	13	NULL	NULL	NULL	AT1-R antagonists	Chemical	treatment	elevates					Ang II	GP	levels of;;plasma			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_12_1182_s_30	null	5 6  Treatment with AT1-R antagonists causes a marked elevation of levels of plasma Ang II, which selectively binds to AT2-R and exerts as yet undefined effects.	bind
28264	2	8324	6	13	NULL	NULL	NULL	Ang II	GP	plasma	bind		selectively			AT2-R	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_12_1182_s_30	null	5 6  Treatment with AT1-R antagonists causes a marked elevation of levels of plasma Ang II, which selectively binds to AT2-R and exerts as yet undefined effects.	bind
34424	1	8324	7	NULL	NULL	0	NULL	Ang II	NULL	plasma	binds to	NULL	selectively			 AT2-R 	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_12_1182_s_30	null	5 6  Treatment with AT1-R antagonists causes a marked elevation of levels of plasma Ang II, which selectively binds to AT2-R and exerts as yet undefined effects.	bind
34425	2	8324	7	10	NULL	0	NULL	AT1-R antagonists	NULL	treatment	elevates	NULL				Ang II	NULL	levels of;;plasma			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_12_1182_s_30	null	5 6  Treatment with AT1-R antagonists causes a marked elevation of levels of plasma Ang II, which selectively binds to AT2-R and exerts as yet undefined effects.	bind
28265	1	8325	6	13	NULL	NULL	NULL	vessel wall	OrganismPart		bind					vWF	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_200_s_28	9484984	5 6 7 8 9 10 11  Because the first event in thrombogenesis is the recognition of vessel wall - bound vWF by platelets through the GPIb receptor, it is apparent that the selective inhibition of binding of endogenous vWF to GPIb may be an appropriate early intervention likely to result in a beneficial antithrombotic effect.	bind
28266	2	8325	6	13	NULL	NULL	NULL	platelets	Cell		recognize					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_200_s_28	9484984	5 6 7 8 9 10 11  Because the first event in thrombogenesis is the recognition of vessel wall - bound vWF by platelets through the GPIb receptor, it is apparent that the selective inhibition of binding of endogenous vWF to GPIb may be an appropriate early intervention likely to result in a beneficial antithrombotic effect.	bind
28267	3	8325	6	13	NULL	NULL	NULL	statement 2	Process		is the first step for					thrombogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_200_s_28	9484984	5 6 7 8 9 10 11  Because the first event in thrombogenesis is the recognition of vessel wall - bound vWF by platelets through the GPIb receptor, it is apparent that the selective inhibition of binding of endogenous vWF to GPIb may be an appropriate early intervention likely to result in a beneficial antithrombotic effect.	bind
28268	4	8325	6	13	NULL	NULL	NULL	statement 2	Process		occurs through					GPIb receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_200_s_28	9484984	5 6 7 8 9 10 11  Because the first event in thrombogenesis is the recognition of vessel wall - bound vWF by platelets through the GPIb receptor, it is apparent that the selective inhibition of binding of endogenous vWF to GPIb may be an appropriate early intervention likely to result in a beneficial antithrombotic effect.	bind
28269	5	8325	6	13	NULL	NULL	NULL	vWF	GP	endogenous	bind					GPIb	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_200_s_28	9484984	5 6 7 8 9 10 11  Because the first event in thrombogenesis is the recognition of vessel wall - bound vWF by platelets through the GPIb receptor, it is apparent that the selective inhibition of binding of endogenous vWF to GPIb may be an appropriate early intervention likely to result in a beneficial antithrombotic effect.	bind
28270	6	8325	6	13	NULL	NULL	NULL	statement 5	Process	inhibition of	results in		may			antithrombotic effect	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_200_s_28	9484984	5 6 7 8 9 10 11  Because the first event in thrombogenesis is the recognition of vessel wall - bound vWF by platelets through the GPIb receptor, it is apparent that the selective inhibition of binding of endogenous vWF to GPIb may be an appropriate early intervention likely to result in a beneficial antithrombotic effect.	bind
34426	1	8325	7	10	NULL	0	NULL	platelets	NULL		recognize	NULL				statement 6	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_200_s_28	9484984	5 6 7 8 9 10 11  Because the first event in thrombogenesis is the recognition of vessel wall - bound vWF by platelets through the GPIb receptor, it is apparent that the selective inhibition of binding of endogenous vWF to GPIb may be an appropriate early intervention likely to result in a beneficial antithrombotic effect.	bind
34427	2	8325	7	NULL	NULL	0	NULL	statement 1	NULL		occurs through	NULL				GPIb receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_200_s_28	9484984	5 6 7 8 9 10 11  Because the first event in thrombogenesis is the recognition of vessel wall - bound vWF by platelets through the GPIb receptor, it is apparent that the selective inhibition of binding of endogenous vWF to GPIb may be an appropriate early intervention likely to result in a beneficial antithrombotic effect.	bind
34428	3	8325	7	NULL	NULL	0	NULL	vWF	NULL	endogenous	bind	NULL				GPIb	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_200_s_28	9484984	5 6 7 8 9 10 11  Because the first event in thrombogenesis is the recognition of vessel wall - bound vWF by platelets through the GPIb receptor, it is apparent that the selective inhibition of binding of endogenous vWF to GPIb may be an appropriate early intervention likely to result in a beneficial antithrombotic effect.	bind
34429	4	8325	7	NULL	NULL	0	NULL	statement 1	NULL		is the first event in	NULL				thrombogenesis	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_200_s_28	9484984	5 6 7 8 9 10 11  Because the first event in thrombogenesis is the recognition of vessel wall - bound vWF by platelets through the GPIb receptor, it is apparent that the selective inhibition of binding of endogenous vWF to GPIb may be an appropriate early intervention likely to result in a beneficial antithrombotic effect.	bind
34430	5	8325	7	NULL	NULL	0	NULL	statement 3	NULL	inhibition of	result in	NULL				antithrombotic effect	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_200_s_28	9484984	5 6 7 8 9 10 11  Because the first event in thrombogenesis is the recognition of vessel wall - bound vWF by platelets through the GPIb receptor, it is apparent that the selective inhibition of binding of endogenous vWF to GPIb may be an appropriate early intervention likely to result in a beneficial antithrombotic effect.	bind
46869	6	8325	7	10	NULL	0	NULL	vessel wall	NULL		bind	NULL				vWF	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_2_200_s_28	9484984	5 6 7 8 9 10 11  Because the first event in thrombogenesis is the recognition of vessel wall - bound vWF by platelets through the GPIb receptor, it is apparent that the selective inhibition of binding of endogenous vWF to GPIb may be an appropriate early intervention likely to result in a beneficial antithrombotic effect.	bind
28271	1	8326	6	13	NULL	NULL	NULL	PC	GP	activation of	occurs via					PC pathway	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2765_s_22	9409254	5 6 7 8 9 10 11  PC activation in vivo occurs via the PC pathway, in which thrombin binds to the endothelial transmembrane protein TM, which acts as a cofactor in accelerating PC activation by thrombin.	bind
28272	2	8326	6	13	NULL	NULL	NULL	thrombin	GP		bind					TM	GP	endothelial			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2765_s_22	9409254	5 6 7 8 9 10 11  PC activation in vivo occurs via the PC pathway, in which thrombin binds to the endothelial transmembrane protein TM, which acts as a cofactor in accelerating PC activation by thrombin.	bind
28273	3	8326	6	13	NULL	NULL	NULL	TM	GP		is a type of					transmembrane protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2765_s_22	9409254	5 6 7 8 9 10 11  PC activation in vivo occurs via the PC pathway, in which thrombin binds to the endothelial transmembrane protein TM, which acts as a cofactor in accelerating PC activation by thrombin.	bind
28274	4	8326	6	13	NULL	NULL	NULL	thrombin	GP		activates					PC	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2765_s_22	9409254	5 6 7 8 9 10 11  PC activation in vivo occurs via the PC pathway, in which thrombin binds to the endothelial transmembrane protein TM, which acts as a cofactor in accelerating PC activation by thrombin.	bind
28275	5	8326	6	13	NULL	NULL	NULL	TM	GP	endothelial	acts as a cofactor for					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2765_s_22	9409254	5 6 7 8 9 10 11  PC activation in vivo occurs via the PC pathway, in which thrombin binds to the endothelial transmembrane protein TM, which acts as a cofactor in accelerating PC activation by thrombin.	bind
34431	1	8326	7	NULL	NULL	0	NULL	PC	NULL	activation of	occurs via	NULL				PC pathway	NULL				NULL	in vivo	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2765_s_22	9409254	5 6 7 8 9 10 11  PC activation in vivo occurs via the PC pathway, in which thrombin binds to the endothelial transmembrane protein TM, which acts as a cofactor in accelerating PC activation by thrombin.	bind
34432	2	8326	7	10	NULL	0	NULL	thrombin	NULL		binds	NULL				TM	NULL	endothelial			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2765_s_22	9409254	5 6 7 8 9 10 11  PC activation in vivo occurs via the PC pathway, in which thrombin binds to the endothelial transmembrane protein TM, which acts as a cofactor in accelerating PC activation by thrombin.	bind
34433	3	8326	7	NULL	NULL	0	NULL	TM	NULL		is a type of	NULL				transmembrane protein	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2765_s_22	9409254	5 6 7 8 9 10 11  PC activation in vivo occurs via the PC pathway, in which thrombin binds to the endothelial transmembrane protein TM, which acts as a cofactor in accelerating PC activation by thrombin.	bind
34434	4	8326	7	NULL	NULL	0	NULL	thrombin	NULL		activates	NULL				PC	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2765_s_22	9409254	5 6 7 8 9 10 11  PC activation in vivo occurs via the PC pathway, in which thrombin binds to the endothelial transmembrane protein TM, which acts as a cofactor in accelerating PC activation by thrombin.	bind
34435	5	8326	7	10	NULL	0	NULL	TM	NULL	endothelial	acts as a	NULL				cofactor	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2765_s_22	9409254	5 6 7 8 9 10 11  PC activation in vivo occurs via the PC pathway, in which thrombin binds to the endothelial transmembrane protein TM, which acts as a cofactor in accelerating PC activation by thrombin.	bind
34436	6	8326	7	NULL	NULL	0	NULL	statement 5	NULL		accelerates	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2765_s_22	9409254	5 6 7 8 9 10 11  PC activation in vivo occurs via the PC pathway, in which thrombin binds to the endothelial transmembrane protein TM, which acts as a cofactor in accelerating PC activation by thrombin.	bind
28276	1	8327	6	13	NULL	NULL	NULL	colchicine	Chemical		bind					tubulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_47_4_451_s_45	11266419	5 Also, two of the compounds used for the present study, compounds  1 and  3, inhibit competitively the binding of colchicine to tubulin and the polymerization of tubulin.	bind
46870	2	8327	6	13	NULL	NULL	NULL	tubulin	GP		undergoes					polymerization	Process				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_47_4_451_s_45	11266419	5 Also, two of the compounds used for the present study, compounds  1 and  3, inhibit competitively the binding of colchicine to tubulin and the polymerization of tubulin.	bind
34437	1	8327	7	NULL	NULL	0	NULL	colchicine	NULL		bind	NULL				tubulin	NULL				NULL		0	NULL	NULL	NULL	gw60_jantimicrobchemoth_47_4_451_s_45	11266419	5 Also, two of the compounds used for the present study, compounds  1 and  3, inhibit competitively the binding of colchicine to tubulin and the polymerization of tubulin.	bind
34438	2	8327	7	NULL	NULL	0	NULL	tubulin 	NULL		undergoes	NULL				polymerization	NULL				NULL		0	NULL	NULL	NULL	gw60_jantimicrobchemoth_47_4_451_s_45	11266419	5 Also, two of the compounds used for the present study, compounds  1 and  3, inhibit competitively the binding of colchicine to tubulin and the polymerization of tubulin.	bind
28277	1	8328	6	13	NULL	NULL	NULL	MP	GP		bind					myosin	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulationres_90_5_546_s_155	11909818	5 Although binding of MP to myosin has been demonstrated in fractionated cells 6 and in vitro, 7 imaging studies of intact cells have raised some questions on this issue.	bind
34439	1	8328	7	NULL	NULL	0	NULL	MP	NULL		bind	NULL				myosin	NULL				NULL	 fractionated cells in vitro	0	NULL	NULL	NULL	gw60_circulationres_90_5_546_s_155	11909818	5 Although binding of MP to myosin has been demonstrated in fractionated cells 6 and in vitro, 7 imaging studies of intact cells have raised some questions on this issue.	bind
28278	1	8330	6	13	NULL	NULL	NULL	ATP	Chemical		bind							isolated	epsilon subunit		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_48_40130_s_226	16203732	5 ATP binding to the isolated epsilon subunit was not affected by lauryldodecylamine oxide ( Kd = 1.4 muM at 35  degrees C).	bind
28279	2	8330	6	13	NULL	NULL	NULL	statement 1	Process		was not affected by					lauryldodecylamine oxide	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_48_40130_s_226	16203732	5 ATP binding to the isolated epsilon subunit was not affected by lauryldodecylamine oxide ( Kd = 1.4 muM at 35  degrees C).	bind
34442	1	8330	7	NULL	NULL	0	NULL	ATP	NULL		bind	NULL					NULL	isolated	epsilon subunit		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_48_40130_s_226	16203732	5 ATP binding to the isolated epsilon subunit was not affected by lauryldodecylamine oxide ( Kd = 1.4 muM at 35  degrees C).	bind
34443	2	8330	7	10	NULL	0	NULL	lauryldodecylamine oxide	NULL		does not affect	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_48_40130_s_226	16203732	5 ATP binding to the isolated epsilon subunit was not affected by lauryldodecylamine oxide ( Kd = 1.4 muM at 35  degrees C).	bind
28281	1	8332	6	13	NULL	NULL	NULL	beta-lactam	GP		bind					BlaR1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_47_4_377_s_13	11266408	5 Binding of a beta-lactam to BlaR1, the signal transducer, is presumed to alter its conformation so that a signal is transmitted across the bacterial membrane and this signal renders BlaI unable to bind to operator DNA, thus allowing transcription of  blaZ, and hence production of beta-lactamase.	bind
28282	2	8332	6	13	NULL	NULL	NULL	BlaI	GP		does not bind					operator DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_47_4_377_s_13	11266408	5 Binding of a beta-lactam to BlaR1, the signal transducer, is presumed to alter its conformation so that a signal is transmitted across the bacterial membrane and this signal renders BlaI unable to bind to operator DNA, thus allowing transcription of  blaZ, and hence production of beta-lactamase.	bind
28283	3	8332	6	13	NULL	NULL	NULL	statement 1	Process		disrupts					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_47_4_377_s_13	11266408	5 Binding of a beta-lactam to BlaR1, the signal transducer, is presumed to alter its conformation so that a signal is transmitted across the bacterial membrane and this signal renders BlaI unable to bind to operator DNA, thus allowing transcription of  blaZ, and hence production of beta-lactamase.	bind
28284	4	8332	6	13	NULL	NULL	NULL	statement 3	Process		allows					blaZ	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_47_4_377_s_13	11266408	5 Binding of a beta-lactam to BlaR1, the signal transducer, is presumed to alter its conformation so that a signal is transmitted across the bacterial membrane and this signal renders BlaI unable to bind to operator DNA, thus allowing transcription of  blaZ, and hence production of beta-lactamase.	bind
28285	5	8332	6	13	NULL	NULL	NULL	statement 4	Process		leads to					beta-lactamase	GP	production of 			NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_47_4_377_s_13	11266408	5 Binding of a beta-lactam to BlaR1, the signal transducer, is presumed to alter its conformation so that a signal is transmitted across the bacterial membrane and this signal renders BlaI unable to bind to operator DNA, thus allowing transcription of  blaZ, and hence production of beta-lactamase.	bind
46871	6	8332	6	13	NULL	NULL	NULL	BlaR1	GP		is a type of					signal transducer	GP				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_47_4_377_s_13	11266408	5 Binding of a beta-lactam to BlaR1, the signal transducer, is presumed to alter its conformation so that a signal is transmitted across the bacterial membrane and this signal renders BlaI unable to bind to operator DNA, thus allowing transcription of  blaZ, and hence production of beta-lactamase.	bind
47087	7	8332	6	13	NULL	NULL	NULL	signal	Process		is transmitted across					bacterial membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_47_4_377_s_13	11266408	5 Binding of a beta-lactam to BlaR1, the signal transducer, is presumed to alter its conformation so that a signal is transmitted across the bacterial membrane and this signal renders BlaI unable to bind to operator DNA, thus allowing transcription of  blaZ, and hence production of beta-lactamase.	bind
47088	8	8332	6	13	NULL	NULL	NULL	statement 7	Process		renders					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_47_4_377_s_13	11266408	5 Binding of a beta-lactam to BlaR1, the signal transducer, is presumed to alter its conformation so that a signal is transmitted across the bacterial membrane and this signal renders BlaI unable to bind to operator DNA, thus allowing transcription of  blaZ, and hence production of beta-lactamase.	bind
47089	9	8332	6	13	NULL	NULL	NULL	statement 1	Process		alter		may			BlaR1	GP	conformation of 			NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_47_4_377_s_13	11266408	5 Binding of a beta-lactam to BlaR1, the signal transducer, is presumed to alter its conformation so that a signal is transmitted across the bacterial membrane and this signal renders BlaI unable to bind to operator DNA, thus allowing transcription of  blaZ, and hence production of beta-lactamase.	bind
34445	1	8332	7	NULL	NULL	0	NULL	beta-lactam	NULL		bind	NULL				BlaR1	NULL				NULL		0	NULL	NULL	NULL	gw60_jantimicrobchemoth_47_4_377_s_13	11266408	5 Binding of a beta-lactam to BlaR1, the signal transducer, is presumed to alter its conformation so that a signal is transmitted across the bacterial membrane and this signal renders BlaI unable to bind to operator DNA, thus allowing transcription of  blaZ, and hence production of beta-lactamase.	bind
34446	2	8332	7	NULL	NULL	0	NULL	BlaR1	NULL		is a type of	NULL				signal transducer	NULL				NULL		0	NULL	NULL	NULL	gw60_jantimicrobchemoth_47_4_377_s_13	11266408	5 Binding of a beta-lactam to BlaR1, the signal transducer, is presumed to alter its conformation so that a signal is transmitted across the bacterial membrane and this signal renders BlaI unable to bind to operator DNA, thus allowing transcription of  blaZ, and hence production of beta-lactamase.	bind
34447	3	8332	7	10	NULL	0	NULL	statement 1	NULL		alters	NULL	may			BlaR1	NULL	conformation of			NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_47_4_377_s_13	11266408	5 Binding of a beta-lactam to BlaR1, the signal transducer, is presumed to alter its conformation so that a signal is transmitted across the bacterial membrane and this signal renders BlaI unable to bind to operator DNA, thus allowing transcription of  blaZ, and hence production of beta-lactamase.	bind
34448	4	8332	7	10	NULL	0	NULL	statement 3	NULL		leads to	NULL				statement 9	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_47_4_377_s_13	11266408	5 Binding of a beta-lactam to BlaR1, the signal transducer, is presumed to alter its conformation so that a signal is transmitted across the bacterial membrane and this signal renders BlaI unable to bind to operator DNA, thus allowing transcription of  blaZ, and hence production of beta-lactamase.	bind
34449	5	8332	7	NULL	NULL	0	NULL	BlaI 	NULL		does not bind	NULL				operator DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jantimicrobchemoth_47_4_377_s_13	11266408	5 Binding of a beta-lactam to BlaR1, the signal transducer, is presumed to alter its conformation so that a signal is transmitted across the bacterial membrane and this signal renders BlaI unable to bind to operator DNA, thus allowing transcription of  blaZ, and hence production of beta-lactamase.	bind
34450	6	8332	7	10	NULL	0	NULL	statement 9	NULL		renders	NULL				statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_47_4_377_s_13	11266408	5 Binding of a beta-lactam to BlaR1, the signal transducer, is presumed to alter its conformation so that a signal is transmitted across the bacterial membrane and this signal renders BlaI unable to bind to operator DNA, thus allowing transcription of  blaZ, and hence production of beta-lactamase.	bind
34451	7	8332	7	NULL	NULL	0	NULL	statement 5	NULL		allows	NULL				blaZ	NULL	transcription of			NULL		0	NULL	NULL	NULL	gw60_jantimicrobchemoth_47_4_377_s_13	11266408	5 Binding of a beta-lactam to BlaR1, the signal transducer, is presumed to alter its conformation so that a signal is transmitted across the bacterial membrane and this signal renders BlaI unable to bind to operator DNA, thus allowing transcription of  blaZ, and hence production of beta-lactamase.	bind
34452	8	8332	7	NULL	NULL	0	NULL	statement 5	NULL		allows	NULL				beta-lactamase	NULL	production of			NULL		0	NULL	NULL	NULL	gw60_jantimicrobchemoth_47_4_377_s_13	11266408	5 Binding of a beta-lactam to BlaR1, the signal transducer, is presumed to alter its conformation so that a signal is transmitted across the bacterial membrane and this signal renders BlaI unable to bind to operator DNA, thus allowing transcription of  blaZ, and hence production of beta-lactamase.	bind
46872	9	8332	7	10	NULL	0	NULL	signal	NULL		is transmitted across	NULL				bacterial membrane	NULL				NULL		0	NULL	NULL	NULL	gw60_jantimicrobchemoth_47_4_377_s_13	11266408	5 Binding of a beta-lactam to BlaR1, the signal transducer, is presumed to alter its conformation so that a signal is transmitted across the bacterial membrane and this signal renders BlaI unable to bind to operator DNA, thus allowing transcription of  blaZ, and hence production of beta-lactamase.	bind
28286	1	8333	6	13	NULL	NULL	NULL	Bruno proteins	GP		bind									BRE element	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_37_28583_s_280	10893231	5 Consistent with the Bruno proteins binding to BRE elements, the  Xenopus EDEN-BP (BrunoL-2) also has been shown to bind to an RNA element that is identical to the consensus BRE ( 26,  60).	bind
28287	2	8333	6	13	NULL	NULL	NULL	EDEN-BP	GP	Xenopus	is					BrunoL-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_37_28583_s_280	10893231	5 Consistent with the Bruno proteins binding to BRE elements, the  Xenopus EDEN-BP (BrunoL-2) also has been shown to bind to an RNA element that is identical to the consensus BRE ( 26,  60).	bind
28288	3	8333	6	13	NULL	NULL	NULL	BrunoL-2	GP	Xenopus	bind									RNA element	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_37_28583_s_280	10893231	5 Consistent with the Bruno proteins binding to BRE elements, the  Xenopus EDEN-BP (BrunoL-2) also has been shown to bind to an RNA element that is identical to the consensus BRE ( 26,  60).	bind
28289	4	8333	6	NULL	NULL	0	NULL		NULL		is identical to	NULL			RNA element		NULL	consensus		BRE	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_37_28583_s_280	10893231	5 Consistent with the Bruno proteins binding to BRE elements, the  Xenopus EDEN-BP (BrunoL-2) also has been shown to bind to an RNA element that is identical to the consensus BRE ( 26,  60).	bind
34453	1	8333	7	NULL	NULL	0	NULL	Bruno proteins	NULL		bind	NULL					NULL			BRE elements	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_37_28583_s_280	10893231	5 Consistent with the Bruno proteins binding to BRE elements, the  Xenopus EDEN-BP (BrunoL-2) also has been shown to bind to an RNA element that is identical to the consensus BRE ( 26,  60).	bind
34454	2	8333	7	NULL	NULL	0	NULL	BrunoL-2	NULL	Xenopus 	bind	NULL					NULL			RNA element	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_37_28583_s_280	10893231	5 Consistent with the Bruno proteins binding to BRE elements, the  Xenopus EDEN-BP (BrunoL-2) also has been shown to bind to an RNA element that is identical to the consensus BRE ( 26,  60).	bind
34455	3	8333	7	10	NULL	0	NULL		NULL		is identical to	NULL			RNA element		NULL	consensus		BRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_37_28583_s_280	10893231	5 Consistent with the Bruno proteins binding to BRE elements, the  Xenopus EDEN-BP (BrunoL-2) also has been shown to bind to an RNA element that is identical to the consensus BRE ( 26,  60).	bind
34456	4	8333	7	NULL	NULL	0	NULL	BrunoL-2	NULL		is	NULL				EDEN-BP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_37_28583_s_280	10893231	5 Consistent with the Bruno proteins binding to BRE elements, the  Xenopus EDEN-BP (BrunoL-2) also has been shown to bind to an RNA element that is identical to the consensus BRE ( 26,  60).	bind
28290	1	8334	6	13	NULL	NULL	NULL	endothelial cells	Cell		secrete					uPA	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
28291	2	8334	6	13	NULL	NULL	NULL	endothelial cells	Cell		secrete					tPA	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
28292	3	8334	6	13	NULL	NULL	NULL	endothelial cells	Cell		secrete					MMP-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
28293	4	8334	6	13	NULL	NULL	NULL	endothelial cells	Cell		secretes					MMP-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
28294	5	8334	6	13	NULL	NULL	NULL	endothelial cells	Cell		secretes					MMP-9	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
28372	6	8334	6	13	NULL	NULL	NULL	uPAR	GP		is					urokinase receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
28373	7	8334	6	13	NULL	NULL	NULL	uPAR	GP		is a type of					membrane-anchored protease receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
28382	8	8334	6	13	NULL	NULL	NULL	proteolytic activity	Process		is restricted to the					cell surface	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
28384	9	8334	6	13	NULL	NULL	NULL	statement 8	Process		occurs via					uPAR	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
28385	10	8334	6	13	NULL	NULL	NULL	statement 8	Process		occurs via					MT1-MMP	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
28386	11	8334	6	13	NULL	NULL	NULL	statement 8	Process		occurs via					MMP-14	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
28387	12	8334	6	13	NULL	NULL	NULL	MT1-MMP	GP		is a type of					membrane type-1 MMP	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
28388	13	8334	6	13	NULL	NULL	NULL	MMP-14	GP		is a type of					membrane type-1 MMP	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
28389	14	8334	6	13	NULL	NULL	NULL	MT1-MMP	GP		bind					uPA	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
28390	15	8334	6	13	NULL	NULL	NULL	MT1-MMP	GP		activate					uPA	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
28392	16	8334	6	13	NULL	NULL	NULL	MMP-14	GP		bind					MMP-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
28393	17	8334	6	13	NULL	NULL	NULL	MMP-14	GP		activate					MMP-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34457	1	8334	7	NULL	NULL	0	NULL	Endothelial cells	NULL		secrete	NULL				uPA	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34458	2	8334	7	NULL	NULL	0	NULL	Endothelial cells	NULL		secrete	NULL				tPA	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34459	3	8334	7	NULL	NULL	0	NULL	Endothelial cells	NULL		secrete	NULL				MMP-1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34460	4	8334	7	NULL	NULL	0	NULL	Endothelial cells	NULL		secrete	NULL				MMP-2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34461	5	8334	7	NULL	NULL	0	NULL	Endothelial cells	NULL		secrete	NULL				MMP-9	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34462	6	8334	7	NULL	NULL	0	NULL	statement 1	NULL		occurs in an	NULL				activation-dependent manner	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34463	7	8334	7	NULL	NULL	0	NULL	statement 2	NULL		occurs in an	NULL				activation-dependent manner	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34464	8	8334	7	NULL	NULL	0	NULL	statement 3	NULL		occurs in an	NULL				activation-dependent manner	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34465	9	8334	7	NULL	NULL	0	NULL	statement 4	NULL		occurs in an	NULL				activation-dependent manner	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34466	10	8334	7	NULL	NULL	0	NULL	statement 5	NULL		occurs in an	NULL				activation-dependent manner	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34467	11	8334	7	NULL	NULL	0	NULL	statement 1	NULL		restrict	NULL				 cell surface proteolytic activity	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34468	12	8334	7	NULL	NULL	0	NULL	statement 2	NULL		restrict	NULL				 cell surface proteolytic activity	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34469	13	8334	7	NULL	NULL	0	NULL	statement 3	NULL		restrict	NULL				cell surface proteolytic activity	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34470	14	8334	7	NULL	NULL	0	NULL	statement 4	NULL		restrict	NULL				cell surface proteolytic activity	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34471	15	8334	7	NULL	NULL	0	NULL	statement 5	NULL		restrict	NULL				cell surface proteolytic activity	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34472	16	8334	7	NULL	NULL	0	NULL	statement 11	NULL		occurs via	NULL				uPAR	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34473	17	8334	7	NULL	NULL	0	NULL	statement 12	NULL		occurs via	NULL				uPAR	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34474	18	8334	7	NULL	NULL	0	NULL	statement 13	NULL		occurs via	NULL				uPAR	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34475	19	8334	7	NULL	NULL	0	NULL	statement 14	NULL		occurs via	NULL				uPAR	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34476	20	8334	7	NULL	NULL	0	NULL	statement 15	NULL		occurs via	NULL				uPAR	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34477	21	8334	7	NULL	NULL	0	NULL	statement 11	NULL		occurs via	NULL				MT1-MMP	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34478	22	8334	7	NULL	NULL	0	NULL	statement 12	NULL		occurs via	NULL				MT1-MMP	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34479	23	8334	7	NULL	NULL	0	NULL	statement 13	NULL		occurs via	NULL				MT1-MMP	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34480	24	8334	7	NULL	NULL	0	NULL	statement 14	NULL		occurs via	NULL				MT1-MMP	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34481	25	8334	7	NULL	NULL	0	NULL	statement 15	NULL		occurs via	NULL				MT1-MMP	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34482	26	8334	7	NULL	NULL	0	NULL	uPAR	NULL		bind	NULL				uPA	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34483	27	8334	7	NULL	NULL	0	NULL	MT1-MMP	NULL		bind	NULL				MMP-2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34484	28	8334	7	NULL	NULL	0	NULL	statement 26	NULL		activate	NULL				uPA	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34485	29	8334	7	NULL	NULL	0	NULL	statement 27	NULL		activate	NULL				MMP-2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34486	30	8334	7	NULL	NULL	0	NULL	uPAR	NULL		is	NULL				urokinase receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34487	31	8334	7	NULL	NULL	0	NULL	MT1-MMP	NULL		is	NULL				membrane type-1 MMP	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34488	32	8334	7	NULL	NULL	0	NULL	MMP-14	NULL		bind	NULL				MMP-2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34489	33	8334	7	NULL	NULL	0	NULL	statement 32	NULL		activate	NULL				MMP-2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34490	34	8334	7	NULL	NULL	0	NULL	uPAR	NULL		is a type of	NULL				membrane-anchored protease receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
34491	35	8334	7	NULL	NULL	0	NULL	MT1-MMP	NULL		is a type of	NULL				membrane-anchored protease receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_106_16_2111_s_21	12379582	5 Endothelial cells secrete uPA, tPA, MMP-1, MMP-2, and MMP-9 in an activation-dependent manner 1, 6 and restrict proteolytic activity to the cell surface via membrane-anchored protease receptors such as urokinase receptor (uPAR) and membrane type-1 MMP (MT1-MMP, MMP-14), which bind and activate uPA and MMP-2, respectively.	bind
28297	1	8336	6	13	NULL	NULL	NULL	flavocytochrome b	GP		bind					p47 phox	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_29_17013_s_118	8663333	5 h after activation of the assay containing p47 phox and p67 phox) almost completely blocked (~91% inhibition) flavocytochrome  b binding to p47 phox compared with controls, supporting the formation of a stable complex that renders the 323-332 binding region inaccessible as was indicated by our peptide studies.	bind
34507	1	8336	7	NULL	NULL	0	NULL	flavocytochrome b	NULL		bind	NULL				p47phox	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_29_17013_s_118	8663333	5 h after activation of the assay containing p47 phox and p67 phox) almost completely blocked (~91% inhibition) flavocytochrome  b binding to p47 phox compared with controls, supporting the formation of a stable complex that renders the 323-332 binding region inaccessible as was indicated by our peptide studies.	bind
28298	1	8337	6	13	NULL	NULL	NULL	VEGFR1	GP		is a type of					tyrosine kinase receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_18_2347_s_27	15867174	5 In ECs, VEGF binds to 2 tyrosine kinase receptors, VEGF receptor (VEGFR) 1 (Flt-1), and VEGFR2 (KDR/Flk1).	bind
28299	2	8337	6	13	NULL	NULL	NULL	VEGFR1	GP		is					VEGF receptor 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_18_2347_s_27	15867174	5 In ECs, VEGF binds to 2 tyrosine kinase receptors, VEGF receptor (VEGFR) 1 (Flt-1), and VEGFR2 (KDR/Flk1).	bind
28300	3	8337	6	13	NULL	NULL	NULL	Flt-1	GP		is a synonym of					VEGFR1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_18_2347_s_27	15867174	5 In ECs, VEGF binds to 2 tyrosine kinase receptors, VEGF receptor (VEGFR) 1 (Flt-1), and VEGFR2 (KDR/Flk1).	bind
28301	4	8337	6	13	NULL	NULL	NULL	KDR/Flk1	GP		is a synonym of					VEGFR2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_18_2347_s_27	15867174	5 In ECs, VEGF binds to 2 tyrosine kinase receptors, VEGF receptor (VEGFR) 1 (Flt-1), and VEGFR2 (KDR/Flk1).	bind
28302	5	8337	6	13	NULL	NULL	NULL	VEGF	GP		bind					VEGFR1	GP				NULL	ECs	NULL	NULL	NULL	NULL	gw70_circulation_111_18_2347_s_27	15867174	5 In ECs, VEGF binds to 2 tyrosine kinase receptors, VEGF receptor (VEGFR) 1 (Flt-1), and VEGFR2 (KDR/Flk1).	bind
28304	6	8337	6	13	NULL	NULL	NULL	VEGF	GP		bind					VEGFR2	GP				NULL	ECs	NULL	NULL	NULL	NULL	gw70_circulation_111_18_2347_s_27	15867174	5 In ECs, VEGF binds to 2 tyrosine kinase receptors, VEGF receptor (VEGFR) 1 (Flt-1), and VEGFR2 (KDR/Flk1).	bind
46873	7	8337	6	13	NULL	NULL	NULL	VEGFR2	GP		is a type of					tyrosine kinase receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_18_2347_s_27	15867174	5 In ECs, VEGF binds to 2 tyrosine kinase receptors, VEGF receptor (VEGFR) 1 (Flt-1), and VEGFR2 (KDR/Flk1).	bind
34512	1	8337	7	10	NULL	0	NULL	VEGFR1	NULL		is a type of	NULL				tyrosine kinase receptor	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_18_2347_s_27	15867174	5 In ECs, VEGF binds to 2 tyrosine kinase receptors, VEGF receptor (VEGFR) 1 (Flt-1), and VEGFR2 (KDR/Flk1).	bind
34513	2	8337	7	10	NULL	0	NULL	VEGF	NULL		bind	NULL				VEGFR1	NULL				NULL	ECs	NULL	NULL	NULL	NULL	gw70_circulation_111_18_2347_s_27	15867174	5 In ECs, VEGF binds to 2 tyrosine kinase receptors, VEGF receptor (VEGFR) 1 (Flt-1), and VEGFR2 (KDR/Flk1).	bind
34514	3	8337	7	NULL	NULL	0	NULL	VEGF	NULL		bind	NULL				VEGFR2	NULL				NULL	ECs	NULL	NULL	NULL	NULL	gw70_circulation_111_18_2347_s_27	15867174	5 In ECs, VEGF binds to 2 tyrosine kinase receptors, VEGF receptor (VEGFR) 1 (Flt-1), and VEGFR2 (KDR/Flk1).	bind
34515	4	8337	7	10	NULL	0	NULL	Flt-1	NULL		is a synonym of	NULL				VEGFR1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_18_2347_s_27	15867174	5 In ECs, VEGF binds to 2 tyrosine kinase receptors, VEGF receptor (VEGFR) 1 (Flt-1), and VEGFR2 (KDR/Flk1).	bind
34516	5	8337	7	10	NULL	0	NULL	KDR/Flk1	NULL		is a synonym of	NULL				VEGFR2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_18_2347_s_27	15867174	5 In ECs, VEGF binds to 2 tyrosine kinase receptors, VEGF receptor (VEGFR) 1 (Flt-1), and VEGFR2 (KDR/Flk1).	bind
34517	6	8337	7	10	NULL	0	NULL	VEGFR1	NULL		is	NULL				VEGF receptor 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_18_2347_s_27	15867174	5 In ECs, VEGF binds to 2 tyrosine kinase receptors, VEGF receptor (VEGFR) 1 (Flt-1), and VEGFR2 (KDR/Flk1).	bind
46874	7	8337	7	10	NULL	0	NULL	VEGFR2	NULL		is a type of	NULL				tyrosine kinase receptor	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_111_18_2347_s_27	15867174	5 In ECs, VEGF binds to 2 tyrosine kinase receptors, VEGF receptor (VEGFR) 1 (Flt-1), and VEGFR2 (KDR/Flk1).	bind
28305	1	8338	6	13	NULL	NULL	NULL	PAR3	GP		bind					thrombin	GP				NULL	mouse platelets	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1640_s_26	16675723	5 In mouse platelets, PAR3 itself does not mediate transmembrane signaling on interaction with thrombin but instead functions as a cofactor that binds thrombin and promotes productive cleavage and activation of PAR4, which then induces intracellular signaling through G-proteins.	bind
28306	2	8338	6	13	NULL	NULL	NULL	PAR3	GP		acts as a cofactor for					statement 1	Process				NULL	mouse platelets	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1640_s_26	16675723	5 In mouse platelets, PAR3 itself does not mediate transmembrane signaling on interaction with thrombin but instead functions as a cofactor that binds thrombin and promotes productive cleavage and activation of PAR4, which then induces intracellular signaling through G-proteins.	bind
28307	3	8338	6	13	NULL	NULL	NULL	statement 2	Process		promotes					PAR4	GP	productive clevage of 			NULL	mouse platelets	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1640_s_26	16675723	5 In mouse platelets, PAR3 itself does not mediate transmembrane signaling on interaction with thrombin but instead functions as a cofactor that binds thrombin and promotes productive cleavage and activation of PAR4, which then induces intracellular signaling through G-proteins.	bind
28308	4	8338	6	13	NULL	NULL	NULL	statement 3	Process		activates					PAR4	GP				NULL	mouse platelets	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1640_s_26	16675723	5 In mouse platelets, PAR3 itself does not mediate transmembrane signaling on interaction with thrombin but instead functions as a cofactor that binds thrombin and promotes productive cleavage and activation of PAR4, which then induces intracellular signaling through G-proteins.	bind
28309	5	8338	6	13	NULL	NULL	NULL	PAR4	GP		induces					intracellular signaling	Process				NULL	mouse platelets	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1640_s_26	16675723	5 In mouse platelets, PAR3 itself does not mediate transmembrane signaling on interaction with thrombin but instead functions as a cofactor that binds thrombin and promotes productive cleavage and activation of PAR4, which then induces intracellular signaling through G-proteins.	bind
28310	6	8338	6	13	NULL	NULL	NULL	statement 5	Process		occurs through					G-proteins	GP				NULL	mouse platelets	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1640_s_26	16675723	5 In mouse platelets, PAR3 itself does not mediate transmembrane signaling on interaction with thrombin but instead functions as a cofactor that binds thrombin and promotes productive cleavage and activation of PAR4, which then induces intracellular signaling through G-proteins.	bind
34521	1	8338	7	10	NULL	0	NULL	PAR3	NULL		bind	NULL				thrombin	NULL				NULL	mouse platelets	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1640_s_26	16675723	5 In mouse platelets, PAR3 itself does not mediate transmembrane signaling on interaction with thrombin but instead functions as a cofactor that binds thrombin and promotes productive cleavage and activation of PAR4, which then induces intracellular signaling through G-proteins.	bind
34522	2	8338	7	NULL	NULL	0	NULL	 PAR3	NULL		does not mediate	NULL				transmembrane signaling	NULL				NULL	mouse platelets	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1640_s_26	16675723	5 In mouse platelets, PAR3 itself does not mediate transmembrane signaling on interaction with thrombin but instead functions as a cofactor that binds thrombin and promotes productive cleavage and activation of PAR4, which then induces intracellular signaling through G-proteins.	bind
34523	3	8338	7	NULL	NULL	0	NULL	statement 2	NULL		occurs upon	NULL				statement 1	NULL				NULL	mouse platelets	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1640_s_26	16675723	5 In mouse platelets, PAR3 itself does not mediate transmembrane signaling on interaction with thrombin but instead functions as a cofactor that binds thrombin and promotes productive cleavage and activation of PAR4, which then induces intracellular signaling through G-proteins.	bind
34524	4	8338	7	10	NULL	0	NULL	PAR3	NULL		acts as a cofactor for	NULL				statement 1	NULL				NULL	mouse platelets	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1640_s_26	16675723	5 In mouse platelets, PAR3 itself does not mediate transmembrane signaling on interaction with thrombin but instead functions as a cofactor that binds thrombin and promotes productive cleavage and activation of PAR4, which then induces intracellular signaling through G-proteins.	bind
34526	5	8338	7	10	NULL	0	NULL	statement 4	NULL		promotes	NULL				PAR4	NULL	productive cleavage of			NULL	mouse platelets	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1640_s_26	16675723	5 In mouse platelets, PAR3 itself does not mediate transmembrane signaling on interaction with thrombin but instead functions as a cofactor that binds thrombin and promotes productive cleavage and activation of PAR4, which then induces intracellular signaling through G-proteins.	bind
34527	6	8338	7	10	NULL	0	NULL	PAR3	NULL		activates	NULL				PAR4	NULL				NULL	mouse platelets	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1640_s_26	16675723	5 In mouse platelets, PAR3 itself does not mediate transmembrane signaling on interaction with thrombin but instead functions as a cofactor that binds thrombin and promotes productive cleavage and activation of PAR4, which then induces intracellular signaling through G-proteins.	bind
34528	7	8338	7	10	NULL	0	NULL	PAR4	NULL		induces	NULL				intracellular signaling	NULL				NULL	mouse platelets	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1640_s_26	16675723	5 In mouse platelets, PAR3 itself does not mediate transmembrane signaling on interaction with thrombin but instead functions as a cofactor that binds thrombin and promotes productive cleavage and activation of PAR4, which then induces intracellular signaling through G-proteins.	bind
34529	8	8338	7	10	NULL	0	NULL	statement 7	NULL		via	NULL				G-proteins	NULL				NULL	mouse platelets	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1640_s_26	16675723	5 In mouse platelets, PAR3 itself does not mediate transmembrane signaling on interaction with thrombin but instead functions as a cofactor that binds thrombin and promotes productive cleavage and activation of PAR4, which then induces intracellular signaling through G-proteins.	bind
28311	1	8339	6	13	NULL	NULL	NULL	HDL3	GP		bind					HSPG	GP	secreted			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulation_108_3_270_s_145	12835223	5 In the present study, PLTP did mediate a modest increase in HDL3 binding to secreted HSPGs in vitro.	bind
28312	2	8339	6	13	NULL	NULL	NULL	PLTP	GP		increases					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulation_108_3_270_s_145	12835223	5 In the present study, PLTP did mediate a modest increase in HDL3 binding to secreted HSPGs in vitro.	bind
34531	1	8339	7	10	NULL	0	NULL	HDL3	NULL		bind	NULL				HSPGs	NULL	secreted			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulation_108_3_270_s_145	12835223	5 In the present study, PLTP did mediate a modest increase in HDL3 binding to secreted HSPGs in vitro.	bind
34532	2	8339	7	NULL	NULL	0	NULL	PLTP	NULL		increase	NULL				statement 1	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulation_108_3_270_s_145	12835223	5 In the present study, PLTP did mediate a modest increase in HDL3 binding to secreted HSPGs in vitro.	bind
28313	1	8340	6	13	NULL	NULL	NULL	PST PIP	GP		bind					PTP HSCF	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_2_989_s_208	9422760	5 Interestingly, the tryptophan located NH2-terminal to the critical tryptophan involved with binding of PST PIP to PTP HSCF does not seem to be required for ligand recognition, a result similar to that found for the NH2-terminal tryptophan of the WW domain in Yes kinase-associated protein ( 14).	bind
34534	1	8340	7	NULL	NULL	0	NULL	PST PIP	NULL		bind	NULL				PTP HSCF	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_2_989_s_208	9422760	5 Interestingly, the tryptophan located NH2-terminal to the critical tryptophan involved with binding of PST PIP to PTP HSCF does not seem to be required for ligand recognition, a result similar to that found for the NH2-terminal tryptophan of the WW domain in Yes kinase-associated protein ( 14).	bind
28405	1	8342	6	13	NULL	NULL	NULL	polyclonal anti-calcitonin antibody	GP	sheep	bind					calcitonin precursor molecules	GP		katacalcin sequence		NULL		NULL	NULL	NULL	NULL	gw70_circulation_109_14_1707_s_42	15066945	5 Kryptor-PCT is based on a sheep polyclonal anti-calcitonin antibody and a monoclonal anti-katacalcin antibody, which bind either to the katacalcin or the calcitonin sequence of calcitonin precursor molecules.	bind
28406	2	8342	6	13	NULL	NULL	NULL	polyclonal anti-calcitonin antibody	GP	sheep	bind					calcitonin precursor molecules	GP		calcitonin sequence		NULL		NULL	NULL	NULL	NULL	gw70_circulation_109_14_1707_s_42	15066945	5 Kryptor-PCT is based on a sheep polyclonal anti-calcitonin antibody and a monoclonal anti-katacalcin antibody, which bind either to the katacalcin or the calcitonin sequence of calcitonin precursor molecules.	bind
28408	3	8342	6	13	NULL	NULL	NULL	anti-katacalcin antibody	GP	monoclonal	bind					calcitonin precursor molecules	GP		katacalcin sequence		NULL		NULL	NULL	NULL	NULL	gw70_circulation_109_14_1707_s_42	15066945	5 Kryptor-PCT is based on a sheep polyclonal anti-calcitonin antibody and a monoclonal anti-katacalcin antibody, which bind either to the katacalcin or the calcitonin sequence of calcitonin precursor molecules.	bind
28409	4	8342	6	13	NULL	NULL	NULL	anti-katacalcin antibody	GP	monoclonal	bind					calcitonin precursor molecules	GP		calcitonin sequence		NULL		NULL	NULL	NULL	NULL	gw70_circulation_109_14_1707_s_42	15066945	5 Kryptor-PCT is based on a sheep polyclonal anti-calcitonin antibody and a monoclonal anti-katacalcin antibody, which bind either to the katacalcin or the calcitonin sequence of calcitonin precursor molecules.	bind
34574	1	8342	7	NULL	NULL	0	NULL	Kryptor-PCT	NULL		is based on	NULL				polyclonal anti-calcitonin antibody	NULL	sheep			NULL		0	NULL	NULL	NULL	gw70_circulation_109_14_1707_s_42	15066945	5 Kryptor-PCT is based on a sheep polyclonal anti-calcitonin antibody and a monoclonal anti-katacalcin antibody, which bind either to the katacalcin or the calcitonin sequence of calcitonin precursor molecules.	bind
34575	2	8342	7	NULL	NULL	0	NULL	Kryptor-PCT 	NULL		is based on	NULL				monoclonal anti-katacalcin antibody	NULL	sheep			NULL		NULL	NULL	NULL	NULL	gw70_circulation_109_14_1707_s_42	15066945	5 Kryptor-PCT is based on a sheep polyclonal anti-calcitonin antibody and a monoclonal anti-katacalcin antibody, which bind either to the katacalcin or the calcitonin sequence of calcitonin precursor molecules.	bind
34576	3	8342	7	10	NULL	0	NULL	Kryptor-PCT	NULL		bind	NULL				katacalcin	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulation_109_14_1707_s_42	15066945	5 Kryptor-PCT is based on a sheep polyclonal anti-calcitonin antibody and a monoclonal anti-katacalcin antibody, which bind either to the katacalcin or the calcitonin sequence of calcitonin precursor molecules.	bind
34577	4	8342	7	NULL	NULL	0	NULL	Kryptor-PCT	NULL		bind	NULL				calcitonin precursor molecules	NULL		calcitonin sequence 		NULL		0	NULL	NULL	NULL	gw70_circulation_109_14_1707_s_42	15066945	5 Kryptor-PCT is based on a sheep polyclonal anti-calcitonin antibody and a monoclonal anti-katacalcin antibody, which bind either to the katacalcin or the calcitonin sequence of calcitonin precursor molecules.	bind
28314	1	8346	6	13	NULL	NULL	NULL	decorin	GP		bind					type VI collagen	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_42_26110_s_137	8824254	5 mug of NG2 inhibits the binding of decorin (0.5 mug) to type VI collagen by only 15%.	bind
28315	2	8346	6	13	NULL	NULL	NULL	NG2	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_42_26110_s_137	8824254	5 mug of NG2 inhibits the binding of decorin (0.5 mug) to type VI collagen by only 15%.	bind
34578	1	8346	7	NULL	NULL	0	NULL	decorin	NULL		bind	NULL				type VI collagen	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_42_26110_s_137	8824254	5 mug of NG2 inhibits the binding of decorin (0.5 mug) to type VI collagen by only 15%.	bind
34579	2	8346	7	NULL	NULL	0	NULL	NG2	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_42_26110_s_137	8824254	5 mug of NG2 inhibits the binding of decorin (0.5 mug) to type VI collagen by only 15%.	bind
28318	1	8353	6	13	NULL	NULL	NULL	B-box proteins	GP	WT	bind					BLT DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_23_16536_s_89	10347218	5 muM amounts of either the correctly folded hybrid or the WT B-box proteins were bound to BLT DNA (0.1 ng) in the footprinting reactions.	bind
34580	1	8353	7	10	NULL	0	NULL	B-box protein	NULL	WT	bind	NULL				BLT DNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_23_16536_s_89	10347218	5 muM amounts of either the correctly folded hybrid or the WT B-box proteins were bound to BLT DNA (0.1 ng) in the footprinting reactions.	bind
47093	1	8354	6	13	NULL	NULL	NULL	18A9	GP		bind					PDHc	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_196	7649984	5 of the 10 MAbs  that bound PDHc (18A9, 21C3, 15A9, 1F2, and 3G1) bound the E1 antigen,  and 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
47097	2	8354	6	13	NULL	NULL	NULL	21C3	GP		bind					PDHc	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_196	7649984	5 of the 10 MAbs  that bound PDHc (18A9, 21C3, 15A9, 1F2, and 3G1) bound the E1 antigen,  and 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
47098	3	8354	6	13	NULL	NULL	NULL	15A9	GP		bind					PDHc	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_196	7649984	5 of the 10 MAbs  that bound PDHc (18A9, 21C3, 15A9, 1F2, and 3G1) bound the E1 antigen,  and 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
47099	4	8354	6	13	NULL	NULL	NULL	1F2 	GP		bind					PDHc	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_196	7649984	5 of the 10 MAbs  that bound PDHc (18A9, 21C3, 15A9, 1F2, and 3G1) bound the E1 antigen,  and 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
47100	5	8354	6	13	NULL	NULL	NULL	3G1 	GP		bind					PDHc	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_196	7649984	5 of the 10 MAbs  that bound PDHc (18A9, 21C3, 15A9, 1F2, and 3G1) bound the E1 antigen,  and 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
47101	6	8354	6	13	NULL	NULL	NULL	18A9	GP		bind					E1 antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_196	7649984	5 of the 10 MAbs  that bound PDHc (18A9, 21C3, 15A9, 1F2, and 3G1) bound the E1 antigen,  and 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
47102	7	8354	6	13	NULL	NULL	NULL	21C3	GP		bind					E1 antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_196	7649984	5 of the 10 MAbs  that bound PDHc (18A9, 21C3, 15A9, 1F2, and 3G1) bound the E1 antigen,  and 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
47103	8	8354	6	13	NULL	NULL	NULL	15A9	GP		bind					E1 antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_196	7649984	5 of the 10 MAbs  that bound PDHc (18A9, 21C3, 15A9, 1F2, and 3G1) bound the E1 antigen,  and 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
47104	9	8354	6	13	NULL	NULL	NULL	1F2	GP		bind					E1 antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_196	7649984	5 of the 10 MAbs  that bound PDHc (18A9, 21C3, 15A9, 1F2, and 3G1) bound the E1 antigen,  and 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
47105	10	8354	6	13	NULL	NULL	NULL	3G1	GP		bind					E1 antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_196	7649984	5 of the 10 MAbs  that bound PDHc (18A9, 21C3, 15A9, 1F2, and 3G1) bound the E1 antigen,  and 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
47106	11	8354	6	13	NULL	NULL	NULL	8C9 	GP		does not bind					E1 antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_196	7649984	5 of the 10 MAbs  that bound PDHc (18A9, 21C3, 15A9, 1F2, and 3G1) bound the E1 antigen,  and 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
47107	12	8354	6	13	NULL	NULL	NULL	7C9	GP		does not bind					E1 antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_196	7649984	5 of the 10 MAbs  that bound PDHc (18A9, 21C3, 15A9, 1F2, and 3G1) bound the E1 antigen,  and 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
47108	13	8354	6	13	NULL	NULL	NULL	13A8	GP		does not bind					E1 antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_196	7649984	5 of the 10 MAbs  that bound PDHc (18A9, 21C3, 15A9, 1F2, and 3G1) bound the E1 antigen,  and 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
47109	14	8354	6	13	NULL	NULL	NULL	23H4	GP		does not bind					E1 antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_196	7649984	5 of the 10 MAbs  that bound PDHc (18A9, 21C3, 15A9, 1F2, and 3G1) bound the E1 antigen,  and 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
47110	15	8354	6	13	NULL	NULL	NULL	8G10	GP		does not bind					E1 antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_196	7649984	5 of the 10 MAbs  that bound PDHc (18A9, 21C3, 15A9, 1F2, and 3G1) bound the E1 antigen,  and 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
34581	1	8354	7	NULL	NULL	0	NULL	18A9 MAb	NULL		bind	NULL				PDHc	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_196	7649984	5 of the 10 MAbs  that bound PDHc (18A9, 21C3, 15A9, 1F2, and 3G1) bound the E1 antigen,  and 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
34582	2	8354	7	NULL	NULL	0	NULL	 21C3 MAb	NULL		bind	NULL				PDHc	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_196	7649984	5 of the 10 MAbs  that bound PDHc (18A9, 21C3, 15A9, 1F2, and 3G1) bound the E1 antigen,  and 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
34583	3	8354	7	NULL	NULL	0	NULL	15A9 MAb	NULL		bind	NULL				PDHc	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_196	7649984	5 of the 10 MAbs  that bound PDHc (18A9, 21C3, 15A9, 1F2, and 3G1) bound the E1 antigen,  and 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
34584	4	8354	7	NULL	NULL	0	NULL	1F2MAb	NULL		bind	NULL				PDHc	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_196	7649984	5 of the 10 MAbs  that bound PDHc (18A9, 21C3, 15A9, 1F2, and 3G1) bound the E1 antigen,  and 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
34585	5	8354	7	NULL	NULL	0	NULL	3G1MAb	NULL		bind	NULL				PDHc	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_196	7649984	5 of the 10 MAbs  that bound PDHc (18A9, 21C3, 15A9, 1F2, and 3G1) bound the E1 antigen,  and 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
34586	6	8354	7	NULL	NULL	0	NULL	18A9 MAb	NULL		bind	NULL				E1 antigen	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_196	7649984	5 of the 10 MAbs  that bound PDHc (18A9, 21C3, 15A9, 1F2, and 3G1) bound the E1 antigen,  and 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
34587	7	8354	7	NULL	NULL	0	NULL	21C3 MAb	NULL		bind	NULL				E1 antigen	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_196	7649984	5 of the 10 MAbs  that bound PDHc (18A9, 21C3, 15A9, 1F2, and 3G1) bound the E1 antigen,  and 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
34588	8	8354	7	NULL	NULL	0	NULL	15A9 MAb	NULL		bind	NULL				E1 antigen	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_196	7649984	5 of the 10 MAbs  that bound PDHc (18A9, 21C3, 15A9, 1F2, and 3G1) bound the E1 antigen,  and 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
34589	9	8354	7	NULL	NULL	0	NULL	1F2MAb	NULL		bind	NULL				E1 antigen	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_196	7649984	5 of the 10 MAbs  that bound PDHc (18A9, 21C3, 15A9, 1F2, and 3G1) bound the E1 antigen,  and 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
34590	10	8354	7	NULL	NULL	0	NULL	3G1MAb	NULL		bind	NULL				E1 antigen	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_196	7649984	5 of the 10 MAbs  that bound PDHc (18A9, 21C3, 15A9, 1F2, and 3G1) bound the E1 antigen,  and 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
34596	11	8354	7	10	NULL	0	NULL	8C9			does not bind					E1 antigen					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_196	7649984	5 of the 10 MAbs  that bound PDHc (18A9, 21C3, 15A9, 1F2, and 3G1) bound the E1 antigen,  and 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
34597	12	8354	7	10	NULL	0	NULL	7C9			does not bind					E1 antigen					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_196	7649984	5 of the 10 MAbs  that bound PDHc (18A9, 21C3, 15A9, 1F2, and 3G1) bound the E1 antigen,  and 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
34598	13	8354	7	10	NULL	0	NULL	13A8			does not bind					E1 antigen					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_196	7649984	5 of the 10 MAbs  that bound PDHc (18A9, 21C3, 15A9, 1F2, and 3G1) bound the E1 antigen,  and 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
34599	14	8354	7	10	NULL	0	NULL	23H4			does not bind					E1 antigen					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_196	7649984	5 of the 10 MAbs  that bound PDHc (18A9, 21C3, 15A9, 1F2, and 3G1) bound the E1 antigen,  and 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
34600	15	8354	7	10	NULL	0	NULL	8G10			does not bind					E1 antigen					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_196	7649984	5 of the 10 MAbs  that bound PDHc (18A9, 21C3, 15A9, 1F2, and 3G1) bound the E1 antigen,  and 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
28319	1	8355	6	13	NULL	NULL	NULL	18A9	GP		bind					E1 antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_152	7649984	5 of these 10 MAbs bound the E1 antigen (18A9, 21C3, 15A9,  1F2, and 3G1), while 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
28320	2	8355	6	13	NULL	NULL	NULL	21C3 MAb	GP		bind					E1 antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_152	7649984	5 of these 10 MAbs bound the E1 antigen (18A9, 21C3, 15A9,  1F2, and 3G1), while 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
28321	3	8355	6	13	NULL	NULL	NULL	15A9 MAb	GP		bind					E1 antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_152	7649984	5 of these 10 MAbs bound the E1 antigen (18A9, 21C3, 15A9,  1F2, and 3G1), while 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
28322	4	8355	6	13	NULL	NULL	NULL	1F2 MAb	GP		bind					E1 antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_152	7649984	5 of these 10 MAbs bound the E1 antigen (18A9, 21C3, 15A9,  1F2, and 3G1), while 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
28323	5	8355	6	13	NULL	NULL	NULL	3G1 MAb	GP		bind					E1 antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_152	7649984	5 of these 10 MAbs bound the E1 antigen (18A9, 21C3, 15A9,  1F2, and 3G1), while 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
28324	6	8355	6	13	NULL	NULL	NULL	8C9 MAb	GP		does not bind					E1 antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_152	7649984	5 of these 10 MAbs bound the E1 antigen (18A9, 21C3, 15A9,  1F2, and 3G1), while 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
28325	7	8355	6	13	NULL	NULL	NULL	7C9	GP		does not bind					E1 antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_152	7649984	5 of these 10 MAbs bound the E1 antigen (18A9, 21C3, 15A9,  1F2, and 3G1), while 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
28326	8	8355	6	13	NULL	NULL	NULL	13A8	GP		does not bind					E1 antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_152	7649984	5 of these 10 MAbs bound the E1 antigen (18A9, 21C3, 15A9,  1F2, and 3G1), while 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
28327	9	8355	6	13	NULL	NULL	NULL	23H4	GP		does not bind					E1 antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_152	7649984	5 of these 10 MAbs bound the E1 antigen (18A9, 21C3, 15A9,  1F2, and 3G1), while 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
28328	10	8355	6	13	NULL	NULL	NULL	8G10	GP		does not bind					E1 antigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_152	7649984	5 of these 10 MAbs bound the E1 antigen (18A9, 21C3, 15A9,  1F2, and 3G1), while 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
34649	1	8355	7	NULL	NULL	0	NULL	18A9 MAb	NULL		bind	NULL				E1 antigen	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_152	7649984	5 of these 10 MAbs bound the E1 antigen (18A9, 21C3, 15A9,  1F2, and 3G1), while 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
34650	2	8355	7	NULL	NULL	0	NULL	21C3 MAb	NULL		bind	NULL				E1 antigen	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_152	7649984	5 of these 10 MAbs bound the E1 antigen (18A9, 21C3, 15A9,  1F2, and 3G1), while 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
34651	3	8355	7	NULL	NULL	0	NULL	15A9 MAb	NULL		bind	NULL				E1 antigen	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_152	7649984	5 of these 10 MAbs bound the E1 antigen (18A9, 21C3, 15A9,  1F2, and 3G1), while 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
34652	4	8355	7	NULL	NULL	0	NULL	 1F2 MAb	NULL		bind	NULL				E1 antigen	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_152	7649984	5 of these 10 MAbs bound the E1 antigen (18A9, 21C3, 15A9,  1F2, and 3G1), while 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
34653	5	8355	7	NULL	NULL	0	NULL	3G1MAb	NULL		bind	NULL				E1 antigen	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_152	7649984	5 of these 10 MAbs bound the E1 antigen (18A9, 21C3, 15A9,  1F2, and 3G1), while 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
34654	6	8355	7	NULL	NULL	0	NULL	8C9 MAb	NULL		does not bind	NULL				E1 antigen	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_152	7649984	5 of these 10 MAbs bound the E1 antigen (18A9, 21C3, 15A9,  1F2, and 3G1), while 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
34655	7	8355	7	NULL	NULL	0	NULL	7C9 MAb	NULL		does not bind	NULL				E1 antigen	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_152	7649984	5 of these 10 MAbs bound the E1 antigen (18A9, 21C3, 15A9,  1F2, and 3G1), while 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
34656	8	8355	7	NULL	NULL	0	NULL	13A8MAb	NULL		does not bind	NULL				E1 antigen	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_152	7649984	5 of these 10 MAbs bound the E1 antigen (18A9, 21C3, 15A9,  1F2, and 3G1), while 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
34657	9	8355	7	NULL	NULL	0	NULL	23H4 MAb	NULL		does not bind	NULL				E1 antigen	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_152	7649984	5 of these 10 MAbs bound the E1 antigen (18A9, 21C3, 15A9,  1F2, and 3G1), while 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
34658	10	8355	7	NULL	NULL	0	NULL	8G10 MAb	NULL		does not bind	NULL				E1 antigen	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19744_s_152	7649984	5 of these 10 MAbs bound the E1 antigen (18A9, 21C3, 15A9,  1F2, and 3G1), while 5 did not (8C9, 7C9, 13A8, 23H4, and 8G10).	bind
28329	1	8356	6	13	NULL	NULL	NULL	L5 protein	GP	rat	bind					5S rRNA	NucleicAcid	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_16_12061_s_130	10766838	5 S rRNA Binding Characteristics of Wild-type and Mutant L5 Proteins-- The binding of rat L5 protein to human 5 S rRNA has been investigated previously ( 29).	bind
34659	1	8356	7	10	NULL	0	NULL	L5 protein	NULL	rat	bind	NULL				5 S rRNA	NULL	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_16_12061_s_130	10766838	5 S rRNA Binding Characteristics of Wild-type and Mutant L5 Proteins-- The binding of rat L5 protein to human 5 S rRNA has been investigated previously ( 29).	bind
28421	1	8358	6	13	NULL	NULL	NULL	5 S rRNA	NucleicAcid		bind					TFIIIA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_47_33198_s_15	10559190	5 S rRNA binds not only to TFIIIA but also to ribosomal protein L5.	bind
28423	2	8358	6	13	NULL	NULL	NULL	5 S rRNA	NucleicAcid		bind					L5 	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_47_33198_s_15	10559190	5 S rRNA binds not only to TFIIIA but also to ribosomal protein L5.	bind
46875	3	8358	6	13	NULL	NULL	NULL	L5	GP		is a type of					ribosomal protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_47_33198_s_15	10559190	5 S rRNA binds not only to TFIIIA but also to ribosomal protein L5.	bind
34661	1	8358	7	NULL	NULL	0	NULL	TFIIIA	NULL		bind	NULL				5 S rRNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_47_33198_s_15	10559190	5 S rRNA binds not only to TFIIIA but also to ribosomal protein L5.	bind
34662	2	8358	7	NULL	NULL	0	NULL	L5	NULL		bind	NULL				5 S rRNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_47_33198_s_15	10559190	5 S rRNA binds not only to TFIIIA but also to ribosomal protein L5.	bind
34663	3	8358	7	NULL	NULL	0	NULL	L5	NULL		is a type of	NULL				ribosomal protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_47_33198_s_15	10559190	5 S rRNA binds not only to TFIIIA but also to ribosomal protein L5.	bind
28426	1	8359	6	13	NULL	NULL	NULL	5 S rRNA gene	NucleicAcid		bind					TFIIIA	GP	partially proteolyzed			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_4_2539_s_150	9891026	5 S rRNA gene binding and transcriptional activation properties of partially proteolyzed TFIIIA.	bind
28427	2	8359	6	13	NULL	NULL	NULL	5 S rRNA gene	NucleicAcid		activates		transcriptionaly			TFIIIA	GP	partially proteolyzed			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_4_2539_s_150	9891026	5 S rRNA gene binding and transcriptional activation properties of partially proteolyzed TFIIIA.	bind
34664	1	8359	7	NULL	NULL	0	NULL	TFIIIA	NULL	partially proteolyzed	bind	NULL				5 S rRNA gene	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_4_2539_s_150	9891026	5 S rRNA gene binding and transcriptional activation properties of partially proteolyzed TFIIIA.	bind
34665	2	8359	7	10	NULL	0	NULL	5 S rRNA gene	NULL		activates	NULL	transcriptionaly 			TFIIIA	NULL	partially proteolyzed			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_4_2539_s_150	9891026	5 S rRNA gene binding and transcriptional activation properties of partially proteolyzed TFIIIA.	bind
28430	1	8360	6	13	NULL	NULL	NULL	rpL1 	GP		bind			carboxyl-terminal 47 amino acids		5S rRNA	NucleicAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_50_30148_s_228	8530422	5 S rRNA-binding Domain in rpL1-HAPrevious  results indicated that a peptide fragment corresponding to the  carboxyl-terminal 47 amino acids of rpL1 can bind 5 S rRNA  in vitro  (Nazar  et al., 1979; Yaguchi  et al., 1984).	bind
34666	1	8360	7	NULL	NULL	0	NULL	rpL1	NULL		bind	NULL		carboxyl-terminal 47 amino acids		5 S rRNA	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_270_50_30148_s_228	8530422	5 S rRNA-binding Domain in rpL1-HAPrevious  results indicated that a peptide fragment corresponding to the  carboxyl-terminal 47 amino acids of rpL1 can bind 5 S rRNA  in vitro  (Nazar  et al., 1979; Yaguchi  et al., 1984).	bind
28432	1	8361	6	13	NULL	NULL	NULL	PN-1	GP	secreted	bind		tightly			ECM	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_1_142_s_19	12524238	5 Secreted PN-1 binds tightly to the extracellular matrix (ECM).	bind
28434	2	8361	6	13	NULL	NULL	NULL	ECM	CellComponent		is					extracellular matrix	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_1_142_s_19	12524238	5 Secreted PN-1 binds tightly to the extracellular matrix (ECM).	bind
34667	1	8361	7	10	NULL	0	NULL	PN-1	NULL	secreted	binds	NULL	tightly			ECM	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_1_142_s_19	12524238	5 Secreted PN-1 binds tightly to the extracellular matrix (ECM).	bind
34668	2	8361	7	NULL	NULL	0	NULL	ECM	NULL		is	NULL				extracellular matrix	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_1_142_s_19	12524238	5 Secreted PN-1 binds tightly to the extracellular matrix (ECM).	bind
28436	1	8362	6	13	NULL	NULL	NULL	Ox-PAPC	Chemical		activates					SREBP	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_768_s_27	16497987	5 SREBP activation by Ox-PAPC was maintained for at least 8 hours, and Ox-PAPC treatment also increased binding of SREBP to a novel SRE sequence in the IL-8 promoter.	bind
28437	2	8362	6	13	NULL	NULL	NULL	SREBP	GP		bind					IL-8	GP			SRE sequence of promoter	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_768_s_27	16497987	5 SREBP activation by Ox-PAPC was maintained for at least 8 hours, and Ox-PAPC treatment also increased binding of SREBP to a novel SRE sequence in the IL-8 promoter.	bind
28438	3	8362	6	13	NULL	NULL	NULL	Ox-PAPC	Chemical	treatment of	increases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_768_s_27	16497987	5 SREBP activation by Ox-PAPC was maintained for at least 8 hours, and Ox-PAPC treatment also increased binding of SREBP to a novel SRE sequence in the IL-8 promoter.	bind
34669	1	8362	7	NULL	NULL	0	NULL	Ox-PAPC	NULL		activates	NULL				SREBP	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_6_768_s_27	16497987	5 SREBP activation by Ox-PAPC was maintained for at least 8 hours, and Ox-PAPC treatment also increased binding of SREBP to a novel SRE sequence in the IL-8 promoter.	bind
34670	2	8362	7	10	NULL	0	NULL	SREBP 	NULL		bind	NULL				IL-8	NULL			SRE sequence of promoter	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_768_s_27	16497987	5 SREBP activation by Ox-PAPC was maintained for at least 8 hours, and Ox-PAPC treatment also increased binding of SREBP to a novel SRE sequence in the IL-8 promoter.	bind
34671	3	8362	7	10	NULL	0	NULL	Ox-PAPC	NULL	treatment	increase	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_768_s_27	16497987	5 SREBP activation by Ox-PAPC was maintained for at least 8 hours, and Ox-PAPC treatment also increased binding of SREBP to a novel SRE sequence in the IL-8 promoter.	bind
28439	1	8363	6	13	NULL	NULL	NULL	heparin	Chemical		bind					antithrombin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_20_20824_s_393	14996843	5 The  Kd value for the binding of heparin to antithrombin was calculated from the quenching of tryptophan fluorescence emission ( closed circles in  Fig. 8).	bind
34672	1	8363	7	NULL	NULL	0	NULL	heparin	NULL		bind	NULL				antithrombin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_20_20824_s_393	14996843	5 The  Kd value for the binding of heparin to antithrombin was calculated from the quenching of tryptophan fluorescence emission ( closed circles in  Fig. 8).	bind
28440	1	8364	6	13	NULL	NULL	NULL	quinidine	Chemical		bind							mutant	E216Q		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_46_38617_s_244	16162505	5 The difference spectra reported here for quinidine binding to the E216Q and E216A mutants appear to be different from those reported by Guengerich  et al. ( ).	bind
28441	2	8364	6	13	NULL	NULL	NULL	quinidine	Chemical		bind							mutant	E216A		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_46_38617_s_244	16162505	5 The difference spectra reported here for quinidine binding to the E216Q and E216A mutants appear to be different from those reported by Guengerich  et al. ( ).	bind
34673	1	8364	7	NULL	NULL	0	NULL	quinidine	NULL		bind	NULL					NULL	mutant	E216Q		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_46_38617_s_244	16162505	5 The difference spectra reported here for quinidine binding to the E216Q and E216A mutants appear to be different from those reported by Guengerich  et al. ( ).	bind
34674	2	8364	7	NULL	NULL	0	NULL	quinidine	NULL		bind	NULL					NULL	mutant	 E216A 		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_46_38617_s_244	16162505	5 The difference spectra reported here for quinidine binding to the E216Q and E216A mutants appear to be different from those reported by Guengerich  et al. ( ).	bind
28442	1	8365	6	13	NULL	NULL	NULL	SRF	GP		is					serum response factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_8_858_s_21	11988486	5 The serum response factor (SRF) binds to the CArG box.	bind
28443	2	8365	6	13	NULL	NULL	NULL	SRF	GP		bind									CArG box	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_8_858_s_21	11988486	5 The serum response factor (SRF) binds to the CArG box.	bind
34675	1	8365	7	NULL	NULL	0	NULL	SRF	NULL		binds to	NULL					NULL			 CArG box	NULL		0	NULL	NULL	NULL	gw60_circulationres_90_8_858_s_21	11988486	5 The serum response factor (SRF) binds to the CArG box.	bind
34676	2	8365	7	NULL	NULL	0	NULL	SRF	NULL		is	NULL				serum response factor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_8_858_s_21	11988486	5 The serum response factor (SRF) binds to the CArG box.	bind
28446	1	8366	6	13	NULL	NULL	NULL	ETF	GP	oxidized	bind					TMADH	GP	oxidized			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_17_12546_s_253	10777543	5 The slight difference seen between the observed and calculated difference spectra is most likely a result of the minor spectral perturbation associated with binding of ETF to TMADH, which is known to occur when the oxidized form of the two proteins bind to each other.	bind
34677	1	8366	7	NULL	NULL	0	NULL	ETF	NULL	Oxidized	bind	NULL				TMADH	NULL	Oxidized			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_17_12546_s_253	10777543	5 The slight difference seen between the observed and calculated difference spectra is most likely a result of the minor spectral perturbation associated with binding of ETF to TMADH, which is known to occur when the oxidized form of the two proteins bind to each other.	bind
28448	1	8367	6	13	NULL	NULL	NULL	MHCI	GP		bind					LILRA5	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_28_19536_s_152	16675463	5 These changes would be likely to inhibit MHCI binding to LILRA5 ( Fig. 3).	bind
34678	1	8367	7	NULL	NULL	0	NULL	MHCI	NULL		bind	NULL				LILRA5	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_28_19536_s_152	16675463	5 These changes would be likely to inhibit MHCI binding to LILRA5 ( Fig. 3).	bind
28449	1	8368	6	13	NULL	NULL	NULL	C-Raf kinase	GP		bind		high affinity			phosphospecific antibody	GP		Ser-621		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_14_14074_s_188	14688280	5 These results reflect a high affinity binding between C-Raf kinase and Ser-621 phosphospecific antibody.	bind
34679	1	8368	7	NULL	NULL	0	NULL	C-Raf kinase	NULL		bind	NULL	high affinity			phosphospecific antibody	NULL		Ser-621		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_14_14074_s_188	14688280	5 These results reflect a high affinity binding between C-Raf kinase and Ser-621 phosphospecific antibody.	bind
28452	1	8369	6	13	NULL	NULL	NULL	Sp1	GP		induces					SMC genes	GP	repression of 			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_981_s_156	15486317	5 These results suggest that Sp1-induced repression of SMC genes may not be a simple function of binding of Sp1 to the G/C repressor and subsequent inhibition of cooperative interactions between CArG elements, as suggested previously by our laboratory.	bind
28454	2	8369	6	13	NULL	NULL	NULL	Sp1	GP		bind									G/C repressor	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_981_s_156	15486317	5 These results suggest that Sp1-induced repression of SMC genes may not be a simple function of binding of Sp1 to the G/C repressor and subsequent inhibition of cooperative interactions between CArG elements, as suggested previously by our laboratory.	bind
34680	1	8369	7	10	NULL	0	NULL	Sp1	NULL		bind	NULL					NULL			G/C repressor	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_981_s_156	15486317	5 These results suggest that Sp1-induced repression of SMC genes may not be a simple function of binding of Sp1 to the G/C repressor and subsequent inhibition of cooperative interactions between CArG elements, as suggested previously by our laboratory.	bind
34681	2	8369	7	NULL	NULL	0	NULL	Sp1	NULL		induce	NULL				SMC genes	NULL	repression of			NULL		0	NULL	NULL	NULL	gw70_circulationres_95_10_981_s_156	15486317	5 These results suggest that Sp1-induced repression of SMC genes may not be a simple function of binding of Sp1 to the G/C repressor and subsequent inhibition of cooperative interactions between CArG elements, as suggested previously by our laboratory.	bind
28456	1	8370	6	13	NULL	NULL	NULL	SHP-1	GP		bind					TCR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_35223_s_134	11435448	5 Unexpectedly, the pace of this SHP-1 binding to the TCR is inversely related to the potency of the TCR ligand used, fast for antagonists and slow for agonists, even though the latter would be expected to be better activators of Lck, enhancing SHP-1 phosphorylation and its recruitment to the TCR.	bind
29018	2	8370	6	13	NULL	NULL	NULL	SHP-1	GP		is recruited to					TCR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_35223_s_134	11435448	5 Unexpectedly, the pace of this SHP-1 binding to the TCR is inversely related to the potency of the TCR ligand used, fast for antagonists and slow for agonists, even though the latter would be expected to be better activators of Lck, enhancing SHP-1 phosphorylation and its recruitment to the TCR.	bind
29019	3	8370	6	13	NULL	NULL	NULL	TCR ligand antagonist	Chemical		increases					statement 1	Process	pace of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_35223_s_134	11435448	5 Unexpectedly, the pace of this SHP-1 binding to the TCR is inversely related to the potency of the TCR ligand used, fast for antagonists and slow for agonists, even though the latter would be expected to be better activators of Lck, enhancing SHP-1 phosphorylation and its recruitment to the TCR.	bind
29020	4	8370	6	13	NULL	NULL	NULL	TCR ligand agonist	Chemical		decreases					statement 1	Process	pace of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_35223_s_134	11435448	5 Unexpectedly, the pace of this SHP-1 binding to the TCR is inversely related to the potency of the TCR ligand used, fast for antagonists and slow for agonists, even though the latter would be expected to be better activators of Lck, enhancing SHP-1 phosphorylation and its recruitment to the TCR.	bind
29021	5	8370	6	13	NULL	NULL	NULL	TCR ligand agonist	Chemical		activates		might			Lck	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_35223_s_134	11435448	5 Unexpectedly, the pace of this SHP-1 binding to the TCR is inversely related to the potency of the TCR ligand used, fast for antagonists and slow for agonists, even though the latter would be expected to be better activators of Lck, enhancing SHP-1 phosphorylation and its recruitment to the TCR.	bind
29022	6	8370	6	13	NULL	NULL	NULL	statement 5	Process		enhances					SHP-1	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_35223_s_134	11435448	5 Unexpectedly, the pace of this SHP-1 binding to the TCR is inversely related to the potency of the TCR ligand used, fast for antagonists and slow for agonists, even though the latter would be expected to be better activators of Lck, enhancing SHP-1 phosphorylation and its recruitment to the TCR.	bind
29023	7	8370	6	13	NULL	NULL	NULL	statement 6	Process		enhances					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_35223_s_134	11435448	5 Unexpectedly, the pace of this SHP-1 binding to the TCR is inversely related to the potency of the TCR ligand used, fast for antagonists and slow for agonists, even though the latter would be expected to be better activators of Lck, enhancing SHP-1 phosphorylation and its recruitment to the TCR.	bind
34683	1	8370	7	NULL	NULL	0	NULL	SHP-1	NULL		bind	NULL				TCR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_38_35223_s_134	11435448	5 Unexpectedly, the pace of this SHP-1 binding to the TCR is inversely related to the potency of the TCR ligand used, fast for antagonists and slow for agonists, even though the latter would be expected to be better activators of Lck, enhancing SHP-1 phosphorylation and its recruitment to the TCR.	bind
34685	3	8370	7	10	NULL	0	NULL	TCR ligand agonists	NULL		activate	NULL				Lck	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_35223_s_134	11435448	5 Unexpectedly, the pace of this SHP-1 binding to the TCR is inversely related to the potency of the TCR ligand used, fast for antagonists and slow for agonists, even though the latter would be expected to be better activators of Lck, enhancing SHP-1 phosphorylation and its recruitment to the TCR.	bind
34686	4	8370	7	NULL	NULL	0	NULL	statement 3	NULL		enhance	NULL				SHP-1	NULL	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_38_35223_s_134	11435448	5 Unexpectedly, the pace of this SHP-1 binding to the TCR is inversely related to the potency of the TCR ligand used, fast for antagonists and slow for agonists, even though the latter would be expected to be better activators of Lck, enhancing SHP-1 phosphorylation and its recruitment to the TCR.	bind
34687	5	8370	7	10	NULL	0	NULL	statement 3	NULL		enhance	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_35223_s_134	11435448	5 Unexpectedly, the pace of this SHP-1 binding to the TCR is inversely related to the potency of the TCR ligand used, fast for antagonists and slow for agonists, even though the latter would be expected to be better activators of Lck, enhancing SHP-1 phosphorylation and its recruitment to the TCR.	bind
46876	2	8370	7	10	NULL	0	NULL	SHP-1	NULL		is recruited to	NULL				TCR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_38_35223_s_134	11435448	5 Unexpectedly, the pace of this SHP-1 binding to the TCR is inversely related to the potency of the TCR ligand used, fast for antagonists and slow for agonists, even though the latter would be expected to be better activators of Lck, enhancing SHP-1 phosphorylation and its recruitment to the TCR.	bind
46877	6	8370	7	10	NULL	0	NULL	TCR ligand antagonist	NULL		increases	NULL				statement 1	NULL	pace of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_38_35223_s_134	11435448	5 Unexpectedly, the pace of this SHP-1 binding to the TCR is inversely related to the potency of the TCR ligand used, fast for antagonists and slow for agonists, even though the latter would be expected to be better activators of Lck, enhancing SHP-1 phosphorylation and its recruitment to the TCR.	bind
46878	7	8370	7	10	NULL	0	NULL	TCR ligand agonist	NULL		decreases	NULL				statement 1	NULL	pace of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_38_35223_s_134	11435448	5 Unexpectedly, the pace of this SHP-1 binding to the TCR is inversely related to the potency of the TCR ligand used, fast for antagonists and slow for agonists, even though the latter would be expected to be better activators of Lck, enhancing SHP-1 phosphorylation and its recruitment to the TCR.	bind
28457	1	8371	6	13	NULL	NULL	NULL	actin capping protein	GP		bind					actin filaments	GP	barbed ends of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_26	14976140	5 Whereas both populations of actin capping protein bind the barbed ends of actin filaments with equal affinities and kinetics 6 the function of beta1-containing actin capping protein is to anchor sarcomeric actin to Z-disc.	bind
28458	2	8371	6	13	NULL	NULL	NULL	actin	GP	sarcomeric	is anchored to					Z-disc	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_26	14976140	5 Whereas both populations of actin capping protein bind the barbed ends of actin filaments with equal affinities and kinetics 6 the function of beta1-containing actin capping protein is to anchor sarcomeric actin to Z-disc.	bind
28459	4	8371	6	13	NULL	NULL	NULL	statement 3	Process		performs					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_26	14976140	5 Whereas both populations of actin capping protein bind the barbed ends of actin filaments with equal affinities and kinetics 6 the function of beta1-containing actin capping protein is to anchor sarcomeric actin to Z-disc.	bind
46883	3	8371	6	13	NULL	NULL	NULL	actin capping protein	GP		contains					beta1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_26	14976140	5 Whereas both populations of actin capping protein bind the barbed ends of actin filaments with equal affinities and kinetics 6 the function of beta1-containing actin capping protein is to anchor sarcomeric actin to Z-disc.	bind
34688	1	8371	7	10	NULL	0	NULL	actin capping protein	NULL		bind	NULL				actin filaments	NULL	barbed ends of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_26	14976140	5 Whereas both populations of actin capping protein bind the barbed ends of actin filaments with equal affinities and kinetics 6 the function of beta1-containing actin capping protein is to anchor sarcomeric actin to Z-disc.	bind
34689	2	8371	7	10	NULL	0	NULL	actin	NULL	sarcomeric	bind	NULL				Z-disc	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_26	14976140	5 Whereas both populations of actin capping protein bind the barbed ends of actin filaments with equal affinities and kinetics 6 the function of beta1-containing actin capping protein is to anchor sarcomeric actin to Z-disc.	bind
34692	4	8371	7	10	NULL	0	NULL	statement 3	NULL		anchor	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_26	14976140	5 Whereas both populations of actin capping protein bind the barbed ends of actin filaments with equal affinities and kinetics 6 the function of beta1-containing actin capping protein is to anchor sarcomeric actin to Z-disc.	bind
46884	3	8371	7	10	NULL	0	NULL	actin capping protein	NULL		contains	NULL				beta1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_3_296_s_26	14976140	5 Whereas both populations of actin capping protein bind the barbed ends of actin filaments with equal affinities and kinetics 6 the function of beta1-containing actin capping protein is to anchor sarcomeric actin to Z-disc.	bind
28460	1	8374	6	13	NULL	NULL	NULL	5' hox genes	GP		is expressed in					epididymis	OrganismPart	adult;; mouse			NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_68_2_644_s_1	12533430	5' hox genes and meis 1, a hox-DNA binding cofactor, are expressed in the adult mouse epididymis.	bind
28461	2	8374	6	13	NULL	NULL	NULL	meis 1	GP		is expressed in					epididymis	OrganismPart	adult;; mouse			NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_68_2_644_s_1	12533430	5' hox genes and meis 1, a hox-DNA binding cofactor, are expressed in the adult mouse epididymis.	bind
28462	3	8374	6	13	NULL	NULL	NULL	meis 1	GP		is a type of					hox-DNA binding cofactor	GP				NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_68_2_644_s_1	12533430	5' hox genes and meis 1, a hox-DNA binding cofactor, are expressed in the adult mouse epididymis.	bind
46885	4	8374	6	13	NULL	NULL	NULL	5' hox genes	GP		is a type of					hox-DNA binding cofactor	GP				NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_68_2_644_s_1	12533430	5' hox genes and meis 1, a hox-DNA binding cofactor, are expressed in the adult mouse epididymis.	bind
34694	1	8374	7	NULL	NULL	0	NULL	5' hox genes	NULL		is a type of	NULL				 hox-DNA binding cofactor	NULL				NULL		0	NULL	NULL	NULL	gw70_biolreprod_68_2_644_s_1	12533430	5' hox genes and meis 1, a hox-DNA binding cofactor, are expressed in the adult mouse epididymis.	bind
34695	2	8374	7	NULL	NULL	0	NULL	meis 1	NULL		is a type of	NULL				hox-DNA binding cofactor	NULL				NULL		0	NULL	NULL	NULL	gw70_biolreprod_68_2_644_s_1	12533430	5' hox genes and meis 1, a hox-DNA binding cofactor, are expressed in the adult mouse epididymis.	bind
34696	3	8374	7	10	NULL	0	NULL	5' hox genes	NULL		is expressed in	NULL				epididymis	NULL	adult;;mouse			NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_68_2_644_s_1	12533430	5' hox genes and meis 1, a hox-DNA binding cofactor, are expressed in the adult mouse epididymis.	bind
34697	4	8374	7	10	NULL	0	NULL	meis 1	NULL		is expressed in	NULL				epididymis	NULL	adult;;mouse			NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_68_2_644_s_1	12533430	5' hox genes and meis 1, a hox-DNA binding cofactor, are expressed in the adult mouse epididymis.	bind
29024	1	8377	6	13	NULL	NULL	NULL	ADP complex	GP		occupies			beta-phosphate					P1 subsite		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_15009_s_256	11154698	5''-ADP complex it is the beta-phosphate rather than the alpha-phosphate that occupies the P1 subsite while the adenosine binds close to the EDN pyrimidine binding subsite B1.	bind
29025	2	8377	6	13	NULL	NULL	NULL	ADP complex	GP		bind			adenosine		EDN 	GP		pyrimidine binding subsite B1		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_15009_s_256	11154698	5''-ADP complex it is the beta-phosphate rather than the alpha-phosphate that occupies the P1 subsite while the adenosine binds close to the EDN pyrimidine binding subsite B1.	bind
34871	1	8377	7	NULL	NULL	0	NULL	 adenosine	NULL		binds	NULL				 EDN	NULL		close to pyrimidine binding subsite B1		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_18_15009_s_256	11154698	5''-ADP complex it is the beta-phosphate rather than the alpha-phosphate that occupies the P1 subsite while the adenosine binds close to the EDN pyrimidine binding subsite B1.	bind
34872	2	8377	7	NULL	NULL	0	NULL	5''-ADP complex	NULL		occupies the	NULL		 beta-phosphate			NULL		P1 subsite		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_18_15009_s_256	11154698	5''-ADP complex it is the beta-phosphate rather than the alpha-phosphate that occupies the P1 subsite while the adenosine binds close to the EDN pyrimidine binding subsite B1.	bind
34873	3	8377	7	NULL	NULL	0	NULL	5''-ADP complex	NULL		does not occupy	NULL		alpha-phosphate			NULL		P1 subsite		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_15009_s_256	11154698	5''-ADP complex it is the beta-phosphate rather than the alpha-phosphate that occupies the P1 subsite while the adenosine binds close to the EDN pyrimidine binding subsite B1.	bind
28463	1	8378	6	13	NULL	NULL	NULL	transcription factor	GP	novel	bind					SR-BI	GP			myeloid zing finger protein-1-like element (-476 to -456) of promoter	NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_j-biol-chem_276_50_11585816_s_11	11585816	5''-Deletion analysis  and gel shift data suggest that LPS inhibits binding of a novel transcription  factor to a myeloid zing finger protein-1-like element (-476 to -456)  in the human SR-BI promoter.	bind
28464	2	8378	6	13	NULL	NULL	NULL	LPS	Chemical		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_j-biol-chem_276_50_11585816_s_11	11585816	5''-Deletion analysis  and gel shift data suggest that LPS inhibits binding of a novel transcription  factor to a myeloid zing finger protein-1-like element (-476 to -456)  in the human SR-BI promoter.	bind
34874	1	8378	7	10	NULL	0	NULL	transcription factor	NULL	novel	bind	NULL				SR-BI 	NULL	human		 myeloid zing finger protein-1-like element -476 to -456 in the promoter	NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_j-biol-chem_276_50_11585816_s_11	11585816	5''-Deletion analysis  and gel shift data suggest that LPS inhibits binding of a novel transcription  factor to a myeloid zing finger protein-1-like element (-476 to -456)  in the human SR-BI promoter.	bind
34875	2	8378	7	NULL	NULL	0	NULL	LPS	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0550-0559_j-biol-chem_276_50_11585816_s_11	11585816	5''-Deletion analysis  and gel shift data suggest that LPS inhibits binding of a novel transcription  factor to a myeloid zing finger protein-1-like element (-476 to -456)  in the human SR-BI promoter.	bind
47526	1	8380	6	13	NULL	NULL	NULL	5''-GTP	Chemical		bind			purine N1 nitrogen		[4Fe - 4] cluster 	GP		Fe site of the C-terminal		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_18_6829_s_98	16632608	5''-GTP binds with its purine N1 nitrogen (2.8- Ang  distance) and its exocyclic amino group (2.4- Ang  distance) in an unprecedented manner to the unique Fe site of the C-terminal [4Fe - 4] cluster ( Fig. 3 A and  C).	bind
47528	2	8380	6	13	NULL	NULL	NULL	5''-GTP	Chemical		bind			exocyclic amino group		[4Fe - 4] cluster	GP		Fe site of the C-terminal		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_18_6829_s_98	16632608	5''-GTP binds with its purine N1 nitrogen (2.8- Ang  distance) and its exocyclic amino group (2.4- Ang  distance) in an unprecedented manner to the unique Fe site of the C-terminal [4Fe - 4] cluster ( Fig. 3 A and  C).	bind
34876	1	8380	7	NULL	NULL	0	NULL	5''-GTP	NULL		bind	NULL		purine N1 nitrogen		 [4Fe - 4] cluster	NULL		unique Fe site of the C-terminal		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_18_6829_s_98	16632608	5''-GTP binds with its purine N1 nitrogen (2.8- Ang  distance) and its exocyclic amino group (2.4- Ang  distance) in an unprecedented manner to the unique Fe site of the C-terminal [4Fe - 4] cluster ( Fig. 3 A and  C).	bind
34878	3	8380	7	NULL	NULL	0	NULL	5''-GTP 	NULL		bind	NULL		exocyclic amino group 		[4Fe - 4] cluster	NULL		unique Fe site of the C-terminal		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_18_6829_s_98	16632608	5''-GTP binds with its purine N1 nitrogen (2.8- Ang  distance) and its exocyclic amino group (2.4- Ang  distance) in an unprecedented manner to the unique Fe site of the C-terminal [4Fe - 4] cluster ( Fig. 3 A and  C).	bind
28545	1	8381	6	13	NULL	NULL	NULL	tau molecule	GP		bind					MTs	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_252	10464280	5) As long as the tau kinases and phosphatases remain in proper balance, the phosphorylation state of tau will remain within limits that favor binding of tau molecules to MTs, as opposed to other tau molecules.	bind
28550	2	8381	6	13	NULL	NULL	NULL	statement 1	Process		is dependent on					tau molecules	GP	phosphorylation state of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_252	10464280	5) As long as the tau kinases and phosphatases remain in proper balance, the phosphorylation state of tau will remain within limits that favor binding of tau molecules to MTs, as opposed to other tau molecules.	bind
34879	1	8381	7	NULL	NULL	0	NULL	 tau molecules	NULL		bind	NULL				MTs	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_252	10464280	5) As long as the tau kinases and phosphatases remain in proper balance, the phosphorylation state of tau will remain within limits that favor binding of tau molecules to MTs, as opposed to other tau molecules.	bind
34880	2	8381	7	NULL	NULL	0	NULL	tau	NULL	 phosphorylation of	favor	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_36_25490_s_252	10464280	5) As long as the tau kinases and phosphatases remain in proper balance, the phosphorylation state of tau will remain within limits that favor binding of tau molecules to MTs, as opposed to other tau molecules.	bind
28559	1	8382	6	13	NULL	NULL	NULL	p47 phox	GP		bind					p22 phox peptides	GP		proline rich		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_13	11733522	5) Binding of both p47 phox and p67 phox to proline-rich p22 phox peptides occurs in the absence of an anionic amphiphile.	bind
28560	2	8382	6	13	NULL	NULL	NULL	p67 phox	GP		bind					p22 phox peptides	GP		proline rich		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_13	11733522	5) Binding of both p47 phox and p67 phox to proline-rich p22 phox peptides occurs in the absence of an anionic amphiphile.	bind
28561	3	8382	6	13	NULL	NULL	NULL	statement 1	Process		occurs in absence of					anionic amphiphile	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_13	11733522	5) Binding of both p47 phox and p67 phox to proline-rich p22 phox peptides occurs in the absence of an anionic amphiphile.	bind
28562	4	8382	6	13	NULL	NULL	NULL	statement 2	Process		occurs in absence of					anionic amphiphile	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_13	11733522	5) Binding of both p47 phox and p67 phox to proline-rich p22 phox peptides occurs in the absence of an anionic amphiphile.	bind
34881	1	8382	7	NULL	NULL	0	NULL	p47 phox 	NULL		bind	NULL				p22 phox peptides	NULL		 proline-rich		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_13	11733522	5) Binding of both p47 phox and p67 phox to proline-rich p22 phox peptides occurs in the absence of an anionic amphiphile.	bind
34882	2	8382	7	NULL	NULL	0	NULL	p67 phox	NULL		bind	NULL				p22 phox peptides	NULL		proline-rich		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_13	11733522	5) Binding of both p47 phox and p67 phox to proline-rich p22 phox peptides occurs in the absence of an anionic amphiphile.	bind
34883	3	8382	7	NULL	NULL	0	NULL	statement 1	NULL		in absence of	NULL				anionic amphiphile	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_13	11733522	5) Binding of both p47 phox and p67 phox to proline-rich p22 phox peptides occurs in the absence of an anionic amphiphile.	bind
34884	4	8382	7	NULL	NULL	0	NULL	statement 2	NULL		in absence of	NULL				anionic amphiphile	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_13	11733522	5) Binding of both p47 phox and p67 phox to proline-rich p22 phox peptides occurs in the absence of an anionic amphiphile.	bind
28563	1	8384	6	13	NULL	NULL	NULL	hsp70	GP		bind					K8/18	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_915_s_209	7529764	5) Binding of hsp70 to K8/18 does not significantly  affect filament assembly  in vitro.	bind
28564	2	8384	6	13	NULL	NULL	NULL	statement 1	Process		does not affect		significantly			filament assembly	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_915_s_209	7529764	5) Binding of hsp70 to K8/18 does not significantly  affect filament assembly  in vitro.	bind
34885	1	8384	7	NULL	NULL	0	NULL	hsp70	NULL		bind	NULL				K8/18	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_270_2_915_s_209	7529764	5) Binding of hsp70 to K8/18 does not significantly  affect filament assembly  in vitro.	bind
34886	2	8384	7	NULL	NULL	0	NULL	statement 1	NULL		does not affect	NULL	significantly			filament assembly	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_270_2_915_s_209	7529764	5) Binding of hsp70 to K8/18 does not significantly  affect filament assembly  in vitro.	bind
28565	1	8385	6	13	NULL	NULL	NULL	InsP(3)R1	GP		bind			SII(+) coupling domain splice variant		AKAP9	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_19375_s_16	14982933	5) Both the SII(+) and the SII(-) coupling domain splice variants of InsP3R1 bind to AKAP9.	bind
28566	2	8385	6	13	NULL	NULL	NULL	InsP(3)R1	GP		bind			SII(-) coupling domain splice variant		AKAP9	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_19375_s_16	14982933	5) Both the SII(+) and the SII(-) coupling domain splice variants of InsP3R1 bind to AKAP9.	bind
34887	1	8385	7	NULL	NULL	0	NULL	InsP3R1	NULL		bind	NULL		SII(+) coupling domain		AKAP9	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_18_19375_s_16	14982933	5) Both the SII(+) and the SII(-) coupling domain splice variants of InsP3R1 bind to AKAP9.	bind
34888	2	8385	7	NULL	NULL	0	NULL	InsP3R1 	NULL		bind	NULL		SII(-) coupling domain		AKAP9	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_18_19375_s_16	14982933	5) Both the SII(+) and the SII(-) coupling domain splice variants of InsP3R1 bind to AKAP9.	bind
28567	1	8386	6	13	NULL	NULL	NULL	ANP	GP		induce		specifically			iNOS mRNA	NucleicAcid	acceleration of;;decay of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_22_13444_s_8	9593677	5) Importantly, two basic mechanisms seem to be responsible for this observation,  i.e. ANP specifically induced acceleration of iNOS mRNA decay and ANP reduced binding activity of NF-kappaB, the transcription factor predominantly responsible for LPS-induced iNOS expression in murine macrophages.	bind
28568	2	8386	6	13	NULL	NULL	NULL	ANP	GP		reduce					NF-kappaB	GP	binding activity of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_22_13444_s_8	9593677	5) Importantly, two basic mechanisms seem to be responsible for this observation,  i.e. ANP specifically induced acceleration of iNOS mRNA decay and ANP reduced binding activity of NF-kappaB, the transcription factor predominantly responsible for LPS-induced iNOS expression in murine macrophages.	bind
28569	3	8386	6	13	NULL	NULL	NULL	NF-kappaB	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_22_13444_s_8	9593677	5) Importantly, two basic mechanisms seem to be responsible for this observation,  i.e. ANP specifically induced acceleration of iNOS mRNA decay and ANP reduced binding activity of NF-kappaB, the transcription factor predominantly responsible for LPS-induced iNOS expression in murine macrophages.	bind
28570	4	8386	6	13	NULL	NULL	NULL	LPS	Chemical		induces					iNOS 	GP	expression of			NULL	murine macrophages	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_22_13444_s_8	9593677	5) Importantly, two basic mechanisms seem to be responsible for this observation,  i.e. ANP specifically induced acceleration of iNOS mRNA decay and ANP reduced binding activity of NF-kappaB, the transcription factor predominantly responsible for LPS-induced iNOS expression in murine macrophages.	bind
28571	5	8386	6	13	NULL	NULL	NULL	NF-kappaB	GP		is responsible for					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_22_13444_s_8	9593677	5) Importantly, two basic mechanisms seem to be responsible for this observation,  i.e. ANP specifically induced acceleration of iNOS mRNA decay and ANP reduced binding activity of NF-kappaB, the transcription factor predominantly responsible for LPS-induced iNOS expression in murine macrophages.	bind
34889	1	8386	7	10	NULL	0	NULL	ANP	NULL		induce	NULL	specifically			iNOS mRNA	NULL	acceleration of;;decay of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_22_13444_s_8	9593677	5) Importantly, two basic mechanisms seem to be responsible for this observation,  i.e. ANP specifically induced acceleration of iNOS mRNA decay and ANP reduced binding activity of NF-kappaB, the transcription factor predominantly responsible for LPS-induced iNOS expression in murine macrophages.	bind
34890	2	8386	7	NULL	NULL	0	NULL	ANP	NULL		reduce	NULL				NF-kappaB	NULL	binding activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_22_13444_s_8	9593677	5) Importantly, two basic mechanisms seem to be responsible for this observation,  i.e. ANP specifically induced acceleration of iNOS mRNA decay and ANP reduced binding activity of NF-kappaB, the transcription factor predominantly responsible for LPS-induced iNOS expression in murine macrophages.	bind
34891	3	8386	7	NULL	NULL	0	NULL	LPS	NULL		induce	NULL				iNOS	NULL	expression of			NULL	murine macrophages	0	NULL	NULL	NULL	gw60_jbiolchem_273_22_13444_s_8	9593677	5) Importantly, two basic mechanisms seem to be responsible for this observation,  i.e. ANP specifically induced acceleration of iNOS mRNA decay and ANP reduced binding activity of NF-kappaB, the transcription factor predominantly responsible for LPS-induced iNOS expression in murine macrophages.	bind
34892	4	8386	7	NULL	NULL	0	NULL	NF-kappaB	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_22_13444_s_8	9593677	5) Importantly, two basic mechanisms seem to be responsible for this observation,  i.e. ANP specifically induced acceleration of iNOS mRNA decay and ANP reduced binding activity of NF-kappaB, the transcription factor predominantly responsible for LPS-induced iNOS expression in murine macrophages.	bind
46891	5	8386	7	10	NULL	0	NULL	NF-kappaB	NULL		is responsible for	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_22_13444_s_8	9593677	5) Importantly, two basic mechanisms seem to be responsible for this observation,  i.e. ANP specifically induced acceleration of iNOS mRNA decay and ANP reduced binding activity of NF-kappaB, the transcription factor predominantly responsible for LPS-induced iNOS expression in murine macrophages.	bind
28572	1	8387	6	13	NULL	NULL	NULL	mannitol	Chemical		bind								C domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_16_12756_s_27	11278734	5) Isothermal titration calorimetry experiments indicated that a significant part of the structural changes upon the binding of mannitol to the C domain reside in the B domain.	bind
34893	1	8387	7	10	NULL	0	NULL	mannitol	NULL		bind	NULL					NULL		C domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_16_12756_s_27	11278734	5) Isothermal titration calorimetry experiments indicated that a significant part of the structural changes upon the binding of mannitol to the C domain reside in the B domain.	bind
28580	1	8388	6	13	NULL	NULL	NULL	FOXO1	GP		bind		directly			PPARgamma2	GP			promoter	NULL	nucleus	NULL	NULL	NULL	NULL	gw70_jbiolchem_281_29_19881_s_286	16670091	5) Once in the nucleus, FOXO1 binds directly to  the PPARgamma2 promoter via at least one specific DNA sequence encompassing bp 270 - 310.	bind
28581	2	8388	6	13	NULL	NULL	NULL	DNA sequence	NucleicAcid		encompass									bp 270 - 310	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_29_19881_s_286	16670091	5) Once in the nucleus, FOXO1 binds directly to  the PPARgamma2 promoter via at least one specific DNA sequence encompassing bp 270 - 310.	bind
56149	3	8388	6	13	NULL	NULL	NULL	statement 1	Process		via					statement 2	Process				NULL	nucleus	NULL	NULL	NULL	NULL	gw70_jbiolchem_281_29_19881_s_286	16670091	5) Once in the nucleus, FOXO1 binds directly to  the PPARgamma2 promoter via at least one specific DNA sequence encompassing bp 270 - 310.	bind
34894	1	8388	7	10	NULL	0	NULL	FOXO1			bind		directly			PPARgamma2				promoter	NULL	nucleus	NULL	NULL	NULL	NULL	gw70_jbiolchem_281_29_19881_s_286	16670091	5) Once in the nucleus, FOXO1 binds directly to  the PPARgamma2 promoter via at least one specific DNA sequence encompassing bp 270 - 310.	bind
56150	2	8388	7	10	NULL	0	NULL	DNA sequence			encompass									bp 270 - 310	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_29_19881_s_286	16670091	5) Once in the nucleus, FOXO1 binds directly to  the PPARgamma2 promoter via at least one specific DNA sequence encompassing bp 270 - 310.	bind
56151	3	8388	7	10	NULL	0	NULL	statement 1			via					statement 2					NULL	nucleus	NULL	NULL	NULL	NULL	gw70_jbiolchem_281_29_19881_s_286	16670091	5) Once in the nucleus, FOXO1 binds directly to  the PPARgamma2 promoter via at least one specific DNA sequence encompassing bp 270 - 310.	bind
28582	1	8389	6	13	NULL	NULL	NULL	p66	GP		bind					apoB RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_44_27700_s_203	9346911	5) p66 and p44, previously characterized as simultaneously binding to apoB RNA, are shown here to have independent RNA cross-linking capabilities.	bind
28583	2	8389	6	13	NULL	NULL	NULL	p44	GP		bind					apoB RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_44_27700_s_203	9346911	5) p66 and p44, previously characterized as simultaneously binding to apoB RNA, are shown here to have independent RNA cross-linking capabilities.	bind
28584	3	8389	6	13	NULL	NULL	NULL	statement 1	Process		occurs simultaneously with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_44_27700_s_203	9346911	5) p66 and p44, previously characterized as simultaneously binding to apoB RNA, are shown here to have independent RNA cross-linking capabilities.	bind
46892	4	8389	6	13	NULL	NULL	NULL	p66	GP		is capable of					RNA cross-linking	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_44_27700_s_203	9346911	5) p66 and p44, previously characterized as simultaneously binding to apoB RNA, are shown here to have independent RNA cross-linking capabilities.	bind
46893	5	8389	6	13	NULL	NULL	NULL	p44	GP		is capable of					RNA cross-linking	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_44_27700_s_203	9346911	5) p66 and p44, previously characterized as simultaneously binding to apoB RNA, are shown here to have independent RNA cross-linking capabilities.	bind
46894	6	8389	6	13	NULL	NULL	NULL	statement 4	Process		is independent of					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_44_27700_s_203	9346911	5) p66 and p44, previously characterized as simultaneously binding to apoB RNA, are shown here to have independent RNA cross-linking capabilities.	bind
34895	1	8389	7	NULL	NULL	0	NULL	p66	NULL		bind	NULL				apoB RNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27700_s_203	9346911	5) p66 and p44, previously characterized as simultaneously binding to apoB RNA, are shown here to have independent RNA cross-linking capabilities.	bind
34896	2	8389	7	NULL	NULL	0	NULL	p44	NULL		bind	NULL				apoB RNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27700_s_203	9346911	5) p66 and p44, previously characterized as simultaneously binding to apoB RNA, are shown here to have independent RNA cross-linking capabilities.	bind
34897	3	8389	7	NULL	NULL	0	NULL	 p66	NULL		capable of	NULL				RNA cross-linking 	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27700_s_203	9346911	5) p66 and p44, previously characterized as simultaneously binding to apoB RNA, are shown here to have independent RNA cross-linking capabilities.	bind
34898	4	8389	7	NULL	NULL	0	NULL	p44	NULL		capable of	NULL				RNA cross-linking 	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27700_s_203	9346911	5) p66 and p44, previously characterized as simultaneously binding to apoB RNA, are shown here to have independent RNA cross-linking capabilities.	bind
46895	5	8389	7	10	NULL	0	NULL	statement 1	NULL		occurs simultaneously with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27700_s_203	9346911	5) p66 and p44, previously characterized as simultaneously binding to apoB RNA, are shown here to have independent RNA cross-linking capabilities.	bind
46896	6	8389	7	10	NULL	0	NULL	statement 3	NULL		is independent of	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27700_s_203	9346911	5) p66 and p44, previously characterized as simultaneously binding to apoB RNA, are shown here to have independent RNA cross-linking capabilities.	bind
28617	1	8390	6	13	NULL	NULL	NULL	Nek6	GP	recombinant	bind		specifically			Nercc1	GP	endogenous			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_37_34897_s_267	12840024	5) Recombinant Nek6 binds to endogenous Nercc1  specifically and in a detergent-resistant manner.	bind
28618	2	8390	6	13	NULL	NULL	NULL	statement 1	Process		is resistant to					detergent	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_37_34897_s_267	12840024	5) Recombinant Nek6 binds to endogenous Nercc1  specifically and in a detergent-resistant manner.	bind
34899	1	8390	7	NULL	NULL	0	NULL	Nek6	NULL	recombinant	binds to	NULL	specifically			Nercc1 	NULL	endogenous			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_34897_s_267	12840024	5) Recombinant Nek6 binds to endogenous Nercc1  specifically and in a detergent-resistant manner.	bind
34900	2	8390	7	NULL	NULL	0	NULL	statement 1	NULL		is resistant to	NULL				detergent	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_34897_s_267	12840024	5) Recombinant Nek6 binds to endogenous Nercc1  specifically and in a detergent-resistant manner.	bind
28620	2	8391	6	13	NULL	NULL	NULL	statement 1	Process		occurs via									DNA sequence that encompasses bp 270 - 310	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_29_19881_s_212	16670091	5) When in the nucleus, FOXO1 binds directly to the PPARgamma2 promoter via a specific DNA sequence that encompasses bp 270 - 310, but probably extends beyond this region (as shown by ChIP).	bind
34901	1	8391	7	NULL	NULL	0	NULL	FOXO1	NULL		binds	NULL	directly			PPARgamma2	NULL			specific DNA sequence that encompasses bp 270 - 310 promoter	NULL	nucleus	NULL	NULL	NULL	NULL	gw70_jbiolchem_281_29_19881_s_212	16670091	5) When in the nucleus, FOXO1 binds directly to the PPARgamma2 promoter via a specific DNA sequence that encompasses bp 270 - 310, but probably extends beyond this region (as shown by ChIP).	bind
28622	1	8394	6	13	NULL	NULL	NULL	rPC	GP		associates with		physically			37-kd laminin receptor precursor	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_5_1447_s_94	11073804	5, 6  rPC is reported to physically associate with 37-kd laminin receptor precursor, which binds to the matrix protein laminin and mediates attachment, differentiation, movement, and growth of the cells.	bind
28623	2	8394	6	13	NULL	NULL	NULL	37-kd laminin receptor precursor	GP		bind					laminin	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_5_1447_s_94	11073804	5, 6  rPC is reported to physically associate with 37-kd laminin receptor precursor, which binds to the matrix protein laminin and mediates attachment, differentiation, movement, and growth of the cells.	bind
28624	3	8394	6	13	NULL	NULL	NULL	laminin	GP		is a type of					matrix protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_5_1447_s_94	11073804	5, 6  rPC is reported to physically associate with 37-kd laminin receptor precursor, which binds to the matrix protein laminin and mediates attachment, differentiation, movement, and growth of the cells.	bind
28625	4	8394	6	13	NULL	NULL	NULL	statement 2	Process		mediates					cells	Cell	attachment of 			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_5_1447_s_94	11073804	5, 6  rPC is reported to physically associate with 37-kd laminin receptor precursor, which binds to the matrix protein laminin and mediates attachment, differentiation, movement, and growth of the cells.	bind
28626	5	8394	6	13	NULL	NULL	NULL	statement 2	Process		mediates					cells	Cell	differentiation of 			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_5_1447_s_94	11073804	5, 6  rPC is reported to physically associate with 37-kd laminin receptor precursor, which binds to the matrix protein laminin and mediates attachment, differentiation, movement, and growth of the cells.	bind
28627	6	8394	6	13	NULL	NULL	NULL	statement 2	Process		mediates					cells	Cell	movement of 			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_5_1447_s_94	11073804	5, 6  rPC is reported to physically associate with 37-kd laminin receptor precursor, which binds to the matrix protein laminin and mediates attachment, differentiation, movement, and growth of the cells.	bind
28628	7	8394	6	13	NULL	NULL	NULL	statement 2	Process		mediates					cells	Cell	growth of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_5_1447_s_94	11073804	5, 6  rPC is reported to physically associate with 37-kd laminin receptor precursor, which binds to the matrix protein laminin and mediates attachment, differentiation, movement, and growth of the cells.	bind
34907	1	8394	7	NULL	NULL	0	NULL	rPC	NULL		associate with	NULL	physically			37-kd laminin receptor precursor	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_5_1447_s_94	11073804	5, 6  rPC is reported to physically associate with 37-kd laminin receptor precursor, which binds to the matrix protein laminin and mediates attachment, differentiation, movement, and growth of the cells.	bind
34908	2	8394	7	NULL	NULL	0	NULL	37-kd laminin receptor precursor	NULL		binds to	NULL				laminin	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_5_1447_s_94	11073804	5, 6  rPC is reported to physically associate with 37-kd laminin receptor precursor, which binds to the matrix protein laminin and mediates attachment, differentiation, movement, and growth of the cells.	bind
34909	3	8394	7	NULL	NULL	0	NULL	laminin	NULL		is a type of	NULL				matrix protein	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_5_1447_s_94	11073804	5, 6  rPC is reported to physically associate with 37-kd laminin receptor precursor, which binds to the matrix protein laminin and mediates attachment, differentiation, movement, and growth of the cells.	bind
34910	4	8394	7	10	NULL	0	NULL	statement 2	NULL		mediates	NULL				cells	NULL	attachment of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_5_1447_s_94	11073804	5, 6  rPC is reported to physically associate with 37-kd laminin receptor precursor, which binds to the matrix protein laminin and mediates attachment, differentiation, movement, and growth of the cells.	bind
34911	5	8394	7	10	NULL	0	NULL	statement 2	NULL		mediates	NULL				cells	NULL	differentiation of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_5_1447_s_94	11073804	5, 6  rPC is reported to physically associate with 37-kd laminin receptor precursor, which binds to the matrix protein laminin and mediates attachment, differentiation, movement, and growth of the cells.	bind
34912	6	8394	7	10	NULL	0	NULL	statement 2	NULL		mediates	NULL				cells	NULL	movement of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_5_1447_s_94	11073804	5, 6  rPC is reported to physically associate with 37-kd laminin receptor precursor, which binds to the matrix protein laminin and mediates attachment, differentiation, movement, and growth of the cells.	bind
34913	7	8394	7	10	NULL	0	NULL	statement 2	NULL		mediates	NULL				cells	NULL	growth of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_5_1447_s_94	11073804	5, 6  rPC is reported to physically associate with 37-kd laminin receptor precursor, which binds to the matrix protein laminin and mediates attachment, differentiation, movement, and growth of the cells.	bind
28629	1	8395	6	13	NULL	NULL	NULL	IGF-1	GP		bind					cell-surface receptor	GP	specific			NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_17_2088_s_22	11673351	5, 6 Binding of IGF-I to its specific cell-surface receptor results in activation of an intracytoplasmatic tyrosin kinase, which phosphorylates insulin receptor substrate-1.	bind
28630	2	8395	6	13	NULL	NULL	NULL	statement 1	Process		results in					tyrosin kinase	GP	activation of;;intracytoplasmatic			NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_17_2088_s_22	11673351	5, 6 Binding of IGF-I to its specific cell-surface receptor results in activation of an intracytoplasmatic tyrosin kinase, which phosphorylates insulin receptor substrate-1.	bind
28631	3	8395	6	13	NULL	NULL	NULL	tyrosin kinase	GP	intracytoplasmatic	phosphorylates					insulin receptor substrate-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_17_2088_s_22	11673351	5, 6 Binding of IGF-I to its specific cell-surface receptor results in activation of an intracytoplasmatic tyrosin kinase, which phosphorylates insulin receptor substrate-1.	bind
34914	1	8395	7	10	NULL	0	NULL	IGF-I	NULL		bind	NULL				cell-surface receptor	NULL	specific			NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_17_2088_s_22	11673351	5, 6 Binding of IGF-I to its specific cell-surface receptor results in activation of an intracytoplasmatic tyrosin kinase, which phosphorylates insulin receptor substrate-1.	bind
34915	2	8395	7	10	NULL	0	NULL	statement 1	NULL		results in	NULL				tyrosine kinase	NULL	activation of;;intracytoplasmatic			NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_17_2088_s_22	11673351	5, 6 Binding of IGF-I to its specific cell-surface receptor results in activation of an intracytoplasmatic tyrosin kinase, which phosphorylates insulin receptor substrate-1.	bind
34916	3	8395	7	NULL	NULL	0	NULL	tyrosin kinase	NULL	intracytoplasmatic	phosphorylates	NULL				 insulin receptor substrate-1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_104_17_2088_s_22	11673351	5, 6 Binding of IGF-I to its specific cell-surface receptor results in activation of an intracytoplasmatic tyrosin kinase, which phosphorylates insulin receptor substrate-1.	bind
28632	1	8396	6	13	NULL	NULL	NULL	IGF-1	GP		prevents					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_10_1220_s_24	11889017	5, 6 Furthermore, IGF-1 prevents apoptosis, 7 and its activity is modulated by IGF-1 binding proteins (IGFBPs), including IGFBP-3.	bind
28633	2	8396	6	13	NULL	NULL	NULL	IGFBP-3	GP		modulate					IGF-1	GP	activity of 			NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_10_1220_s_24	11889017	5, 6 Furthermore, IGF-1 prevents apoptosis, 7 and its activity is modulated by IGF-1 binding proteins (IGFBPs), including IGFBP-3.	bind
28634	3	8396	6	13	NULL	NULL	NULL	IGFBP-3	GP		is a type of					IGF-1 binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_10_1220_s_24	11889017	5, 6 Furthermore, IGF-1 prevents apoptosis, 7 and its activity is modulated by IGF-1 binding proteins (IGFBPs), including IGFBP-3.	bind
46897	4	8396	6	13	NULL	NULL	NULL	IGFBPs	GP		is					IGF-1 binding proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_10_1220_s_24	11889017	5, 6 Furthermore, IGF-1 prevents apoptosis, 7 and its activity is modulated by IGF-1 binding proteins (IGFBPs), including IGFBP-3.	bind
34917	1	8396	7	NULL	NULL	0	NULL	IGF-1	NULL		prevents	NULL				apoptosis	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_10_1220_s_24	11889017	5, 6 Furthermore, IGF-1 prevents apoptosis, 7 and its activity is modulated by IGF-1 binding proteins (IGFBPs), including IGFBP-3.	bind
34918	2	8396	7	10	NULL	0	NULL	IGFBP-3			modulates					IGF-1		activity of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_105_10_1220_s_24	11889017	5, 6 Furthermore, IGF-1 prevents apoptosis, 7 and its activity is modulated by IGF-1 binding proteins (IGFBPs), including IGFBP-3.	bind
34919	3	8396	7	NULL	NULL	0	NULL	IGFBP-3	NULL		is a type of	NULL				IGFBPs	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_10_1220_s_24	11889017	5, 6 Furthermore, IGF-1 prevents apoptosis, 7 and its activity is modulated by IGF-1 binding proteins (IGFBPs), including IGFBP-3.	bind
34920	4	8396	7	NULL	NULL	0	NULL	IGFBPs	NULL		is	NULL				IGF-1 binding proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_105_10_1220_s_24	11889017	5, 6 Furthermore, IGF-1 prevents apoptosis, 7 and its activity is modulated by IGF-1 binding proteins (IGFBPs), including IGFBP-3.	bind
28635	1	8397	6	13	NULL	NULL	NULL	VEGF-D	GP		bind					VEGFR-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_2_395_s_16	9708800	5, 6, 10- 15  The recently identified specific receptor for VEGF-B is VEGFR-1 (B. Olofsson et al, manuscript in preparation), whereas VEGF-D binds both VEGFR-2 and VEGFR-3.	bind
28636	2	8397	6	13	NULL	NULL	NULL	VEGF-D	GP		bind					VEGFR-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_2_395_s_16	9708800	5, 6, 10- 15  The recently identified specific receptor for VEGF-B is VEGFR-1 (B. Olofsson et al, manuscript in preparation), whereas VEGF-D binds both VEGFR-2 and VEGFR-3.	bind
28637	3	8397	6	13	NULL	NULL	NULL	VEGFR-1	GP		is the receptor for					VEGF-B	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_2_395_s_16	9708800	5, 6, 10- 15  The recently identified specific receptor for VEGF-B is VEGFR-1 (B. Olofsson et al, manuscript in preparation), whereas VEGF-D binds both VEGFR-2 and VEGFR-3.	bind
34921	1	8397	7	NULL	NULL	0	NULL	VEGF-B	NULL		bind	NULL	specifically			VEGFR-1	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_2_395_s_16	9708800	5, 6, 10- 15  The recently identified specific receptor for VEGF-B is VEGFR-1 (B. Olofsson et al, manuscript in preparation), whereas VEGF-D binds both VEGFR-2 and VEGFR-3.	bind
34922	2	8397	7	NULL	NULL	0	NULL	VEGF-D	NULL		bind	NULL				VEGFR-2	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_2_395_s_16	9708800	5, 6, 10- 15  The recently identified specific receptor for VEGF-B is VEGFR-1 (B. Olofsson et al, manuscript in preparation), whereas VEGF-D binds both VEGFR-2 and VEGFR-3.	bind
34923	3	8397	7	NULL	NULL	0	NULL	VEGF-D 	NULL		bind	NULL				VEGFR-3	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_2_395_s_16	9708800	5, 6, 10- 15  The recently identified specific receptor for VEGF-B is VEGFR-1 (B. Olofsson et al, manuscript in preparation), whereas VEGF-D binds both VEGFR-2 and VEGFR-3.	bind
28638	1	8398	6	13	NULL	NULL	NULL	SOCS1	GP		is recruited to			SH2 domain		Cbp	GP	phosphorylated	Tyr314		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_42_31920_s_266	16920712	5, the SH2 domain of SOCS1 is recruited to phosphorylated Tyr314 of Cbp.  6, SOCS1 mediates polyubiquitination and proteasomal degradation of Lyn.	bind
28639	2	8398	6	13	NULL	NULL	NULL	SOCS1	GP		mediates					Lyn	GP	polyubiquitination of 			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_42_31920_s_266	16920712	5, the SH2 domain of SOCS1 is recruited to phosphorylated Tyr314 of Cbp.  6, SOCS1 mediates polyubiquitination and proteasomal degradation of Lyn.	bind
28640	3	8398	6	13	NULL	NULL	NULL	SOCS1	GP		mediates					Lyn	GP	proteasomal degradation of 			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_42_31920_s_266	16920712	5, the SH2 domain of SOCS1 is recruited to phosphorylated Tyr314 of Cbp.  6, SOCS1 mediates polyubiquitination and proteasomal degradation of Lyn.	bind
34924	1	8398	7	NULL	NULL	0	NULL	SOCS1	NULL		is recruited to	NULL		SH2 domain		Cbp	NULL	 phosphorylated	Tyr314		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_42_31920_s_266	16920712	5, the SH2 domain of SOCS1 is recruited to phosphorylated Tyr314 of Cbp.  6, SOCS1 mediates polyubiquitination and proteasomal degradation of Lyn.	bind
34925	2	8398	7	10	NULL	0	NULL	SOCS1	NULL		mediates	NULL				Lyn	NULL	polyubiquitination of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_42_31920_s_266	16920712	5, the SH2 domain of SOCS1 is recruited to phosphorylated Tyr314 of Cbp.  6, SOCS1 mediates polyubiquitination and proteasomal degradation of Lyn.	bind
34926	3	8398	7	NULL	NULL	0	NULL	 SOCS1	NULL		mediates	NULL				Lyn	NULL	proteasomal degradation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_42_31920_s_266	16920712	5, the SH2 domain of SOCS1 is recruited to phosphorylated Tyr314 of Cbp.  6, SOCS1 mediates polyubiquitination and proteasomal degradation of Lyn.	bind
28641	1	8399	6	13	NULL	NULL	NULL	Fe3+	Chemical		bind					adenine N7	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_43_42495_s_181	12913009	5, whereas binding of Fe3+ to the adenine N7 is favored at neutral pH ( ).	bind
34927	1	8399	7	NULL	NULL	0	NULL	Fe3+	NULL		bind	NULL				adenine N7	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_43_42495_s_181	12913009	5, whereas binding of Fe3+ to the adenine N7 is favored at neutral pH ( ).	bind
28642	1	8400	6	13	NULL	NULL	NULL	Bcl-2	GP		is localized to					outer mitochondrial membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_21	15345651	5,10,11   Bcl-2 is localized to the outer mitochondrial membrane and Bcl-2 family proteins have been reported to interact with VDAC. 5,7  There is controversy as to whether Bcl-2 binding to VDAC promotes the opening or closing of VDAC. 10,13  Thompson and coworkers 8,10  report that Bcl-2 maintains VDAC in an open state, whereas Shimizu et al 5,11,13   report that Bcl-2 promotes VDAC closure.	bind
28643	2	8400	6	13	NULL	NULL	NULL	Bcl-2 family proteins	GP		interact with					VDAC	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_21	15345651	5,10,11   Bcl-2 is localized to the outer mitochondrial membrane and Bcl-2 family proteins have been reported to interact with VDAC. 5,7  There is controversy as to whether Bcl-2 binding to VDAC promotes the opening or closing of VDAC. 10,13  Thompson and coworkers 8,10  report that Bcl-2 maintains VDAC in an open state, whereas Shimizu et al 5,11,13   report that Bcl-2 promotes VDAC closure.	bind
46900	3	8400	6	13	NULL	NULL	NULL	Bcl-2	GP		maintains					VDAC	GP	open state of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_21	15345651	5,10,11   Bcl-2 is localized to the outer mitochondrial membrane and Bcl-2 family proteins have been reported to interact with VDAC. 5,7  There is controversy as to whether Bcl-2 binding to VDAC promotes the opening or closing of VDAC. 10,13  Thompson and coworkers 8,10  report that Bcl-2 maintains VDAC in an open state, whereas Shimizu et al 5,11,13   report that Bcl-2 promotes VDAC closure.	bind
46901	4	8400	6	13	NULL	NULL	NULL	Bcl-2	GP		promotes					VDAC	GP	closure of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_21	15345651	5,10,11   Bcl-2 is localized to the outer mitochondrial membrane and Bcl-2 family proteins have been reported to interact with VDAC. 5,7  There is controversy as to whether Bcl-2 binding to VDAC promotes the opening or closing of VDAC. 10,13  Thompson and coworkers 8,10  report that Bcl-2 maintains VDAC in an open state, whereas Shimizu et al 5,11,13   report that Bcl-2 promotes VDAC closure.	bind
34929	1	8400	7	NULL	NULL	0	NULL	Bcl-2	NULL		is localized to	NULL				outer mitochondrial membrane	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_21	15345651	5,10,11   Bcl-2 is localized to the outer mitochondrial membrane and Bcl-2 family proteins have been reported to interact with VDAC. 5,7  There is controversy as to whether Bcl-2 binding to VDAC promotes the opening or closing of VDAC. 10,13  Thompson and coworkers 8,10  report that Bcl-2 maintains VDAC in an open state, whereas Shimizu et al 5,11,13   report that Bcl-2 promotes VDAC closure.	bind
34930	2	8400	7	NULL	NULL	0	NULL	Bcl-2 family proteins	NULL		interacts with	NULL				VDAC	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_21	15345651	5,10,11   Bcl-2 is localized to the outer mitochondrial membrane and Bcl-2 family proteins have been reported to interact with VDAC. 5,7  There is controversy as to whether Bcl-2 binding to VDAC promotes the opening or closing of VDAC. 10,13  Thompson and coworkers 8,10  report that Bcl-2 maintains VDAC in an open state, whereas Shimizu et al 5,11,13   report that Bcl-2 promotes VDAC closure.	bind
34931	3	8400	7	10	NULL	0	NULL	Bcl-2	NULL		maintains	NULL				VDAC	NULL	open state of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_21	15345651	5,10,11   Bcl-2 is localized to the outer mitochondrial membrane and Bcl-2 family proteins have been reported to interact with VDAC. 5,7  There is controversy as to whether Bcl-2 binding to VDAC promotes the opening or closing of VDAC. 10,13  Thompson and coworkers 8,10  report that Bcl-2 maintains VDAC in an open state, whereas Shimizu et al 5,11,13   report that Bcl-2 promotes VDAC closure.	bind
46899	4	8400	7	10	NULL	0	NULL	Bcl-2	NULL		promotes	NULL				VDAC	NULL	closure of			NULL		0	NULL	NULL	NULL	gw70_circulationres_95_7_734_s_21	15345651	5,10,11   Bcl-2 is localized to the outer mitochondrial membrane and Bcl-2 family proteins have been reported to interact with VDAC. 5,7  There is controversy as to whether Bcl-2 binding to VDAC promotes the opening or closing of VDAC. 10,13  Thompson and coworkers 8,10  report that Bcl-2 maintains VDAC in an open state, whereas Shimizu et al 5,11,13   report that Bcl-2 promotes VDAC closure.	bind
34802	1	8401	5	13	NULL	NULL	NULL	actin	GP		bind					eNOS	GP			3'UTR	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_5_488_s_214	15256481	5,10,39   Shear stress did not significantly affect actin binding to the eNOS 3'UTR, but treatment with H2O2 resulted in a dramatic decrease in binding activity (online Figure II).	bind
34803	2	8401	5	13	NULL	NULL	NULL	shear stress			does not affect		significantly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_5_488_s_214	15256481	5,10,39   Shear stress did not significantly affect actin binding to the eNOS 3'UTR, but treatment with H2O2 resulted in a dramatic decrease in binding activity (online Figure II).	bind
34804	3	8401	5	13	NULL	NULL	NULL	H2O2	Chemical	treatment	decrease		dramatically			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_5_488_s_214	15256481	5,10,39   Shear stress did not significantly affect actin binding to the eNOS 3'UTR, but treatment with H2O2 resulted in a dramatic decrease in binding activity (online Figure II).	bind
28644	1	8401	6	NULL	NULL	0	NULL	actin	NULL		bind	NULL				eNOS	NULL			3'UTR	NULL		0	NULL	NULL	NULL	gw70_circulationres_95_5_488_s_214	15256481	5,10,39   Shear stress did not significantly affect actin binding to the eNOS 3'UTR, but treatment with H2O2 resulted in a dramatic decrease in binding activity (online Figure II).	bind
28645	2	8401	6	10	NULL	0	NULL	H2O2		treatment	decrease		dramatically			statement 1					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_5_488_s_214	15256481	5,10,39   Shear stress did not significantly affect actin binding to the eNOS 3'UTR, but treatment with H2O2 resulted in a dramatic decrease in binding activity (online Figure II).	bind
28646	3	8401	6	NULL	NULL	0	NULL	shear stress	NULL		did not affect	NULL	significantly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_95_5_488_s_214	15256481	5,10,39   Shear stress did not significantly affect actin binding to the eNOS 3'UTR, but treatment with H2O2 resulted in a dramatic decrease in binding activity (online Figure II).	bind
34805	1	8402	5	13	NULL	NULL	NULL	Sp1	GP		bind					SMMHC	GP			G/C repressor	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_981_s_128	15486317	5,14,15   However, we further demonstrated that Sp1 binding to the SMMHC G/C repressor did not prevent SRF binding to the adjacent CArG2, which is separated from the G/C repressor by 6 nucleotides 14 ( Figure 6a).	bind
34807	2	8402	5	13	NULL	NULL	NULL	SMMHC	GP		is separated from				CArG2	SMMHC	GP			G/C repressor	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_981_s_128	15486317	5,14,15   However, we further demonstrated that Sp1 binding to the SMMHC G/C repressor did not prevent SRF binding to the adjacent CArG2, which is separated from the G/C repressor by 6 nucleotides 14 ( Figure 6a).	bind
34808	3	8402	5	13	NULL	NULL	NULL	nucleotides	NucleicAcid		separate					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_981_s_128	15486317	5,14,15   However, we further demonstrated that Sp1 binding to the SMMHC G/C repressor did not prevent SRF binding to the adjacent CArG2, which is separated from the G/C repressor by 6 nucleotides 14 ( Figure 6a).	bind
34809	4	8402	5	13	NULL	NULL	NULL	SRF	GP		bind					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_981_s_128	15486317	5,14,15   However, we further demonstrated that Sp1 binding to the SMMHC G/C repressor did not prevent SRF binding to the adjacent CArG2, which is separated from the G/C repressor by 6 nucleotides 14 ( Figure 6a).	bind
34810	5	8402	5	13	NULL	NULL	NULL	statement 1	Process		does not prevent					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_981_s_128	15486317	5,14,15   However, we further demonstrated that Sp1 binding to the SMMHC G/C repressor did not prevent SRF binding to the adjacent CArG2, which is separated from the G/C repressor by 6 nucleotides 14 ( Figure 6a).	bind
28647	1	8402	6	NULL	NULL	0	NULL	Sp1	NULL		bind	NULL				SMMHC	NULL			G/C repressor	NULL		0	NULL	NULL	NULL	gw70_circulationres_95_10_981_s_128	15486317	5,14,15   However, we further demonstrated that Sp1 binding to the SMMHC G/C repressor did not prevent SRF binding to the adjacent CArG2, which is separated from the G/C repressor by 6 nucleotides 14 ( Figure 6a).	bind
28648	2	8402	6	10	NULL	0	NULL	SRF			bind					SMMHC				CArG2	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_981_s_128	15486317	5,14,15   However, we further demonstrated that Sp1 binding to the SMMHC G/C repressor did not prevent SRF binding to the adjacent CArG2, which is separated from the G/C repressor by 6 nucleotides 14 ( Figure 6a).	bind
28649	3	8402	6	NULL	NULL	0	NULL	statement 1	NULL		did not prevent	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_95_10_981_s_128	15486317	5,14,15   However, we further demonstrated that Sp1 binding to the SMMHC G/C repressor did not prevent SRF binding to the adjacent CArG2, which is separated from the G/C repressor by 6 nucleotides 14 ( Figure 6a).	bind
28650	4	8402	6	10	NULL	0	NULL	SMMHC			is separated from				CArG2	SMMHC				G/C repressor	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_981_s_128	15486317	5,14,15   However, we further demonstrated that Sp1 binding to the SMMHC G/C repressor did not prevent SRF binding to the adjacent CArG2, which is separated from the G/C repressor by 6 nucleotides 14 ( Figure 6a).	bind
34811	1	8403	5	13	NULL	NULL	NULL	Fos protein	GP		bind					Jun protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2808_s_23	9409259	5,6 In vitro studies have demonstrated that Fos and Jun proteins combine to form stable AP-1 heterodimers, which bind to AP-1 consensus sequences present in numerous genes associated with cell proliferative response and extracellular matrix production.	bind
34812	2	8403	5	13	NULL	NULL	NULL	statement 1	GP		forms					AP-1 heterodimers	GP	stable			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2808_s_23	9409259	5,6 In vitro studies have demonstrated that Fos and Jun proteins combine to form stable AP-1 heterodimers, which bind to AP-1 consensus sequences present in numerous genes associated with cell proliferative response and extracellular matrix production.	bind
35852	3	8403	5	13	NULL	NULL	NULL	AP-1 heterodimers	GP		bind					genes associated with cell proliferative response	GP			AP-1 consensus sequences	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2808_s_23	9409259	5,6 In vitro studies have demonstrated that Fos and Jun proteins combine to form stable AP-1 heterodimers, which bind to AP-1 consensus sequences present in numerous genes associated with cell proliferative response and extracellular matrix production.	bind
35854	4	8403	5	13	NULL	NULL	NULL	AP-1 heterodimers	GP		bind					genes associated with extracellular matrix production	GP			AP-1 consensus sequences	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2808_s_23	9409259	5,6 In vitro studies have demonstrated that Fos and Jun proteins combine to form stable AP-1 heterodimers, which bind to AP-1 consensus sequences present in numerous genes associated with cell proliferative response and extracellular matrix production.	bind
28651	1	8403	6	NULL	NULL	0	NULL	Fox protein	NULL		combine with	NULL				Jun protein	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2808_s_23	9409259	5,6 In vitro studies have demonstrated that Fos and Jun proteins combine to form stable AP-1 heterodimers, which bind to AP-1 consensus sequences present in numerous genes associated with cell proliferative response and extracellular matrix production.	bind
28652	2	8403	6	NULL	NULL	0	NULL	statement 1	NULL		form stable complex with	NULL				AP-1 heterodimers	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2808_s_23	9409259	5,6 In vitro studies have demonstrated that Fos and Jun proteins combine to form stable AP-1 heterodimers, which bind to AP-1 consensus sequences present in numerous genes associated with cell proliferative response and extracellular matrix production.	bind
29027	3	8403	6	NULL	NULL	0	NULL	AP-1 heterodimers	NULL		bind	NULL				gene associated with cell proliferative response	NULL			AP-1 consensus site	NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2808_s_23	9409259	5,6 In vitro studies have demonstrated that Fos and Jun proteins combine to form stable AP-1 heterodimers, which bind to AP-1 consensus sequences present in numerous genes associated with cell proliferative response and extracellular matrix production.	bind
29028	4	8403	6	NULL	NULL	0	NULL	AP-1 heterodimers	NULL		bind	NULL				genes associated with extracellular matrix production	NULL			AP-1 consensus site	NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2808_s_23	9409259	5,6 In vitro studies have demonstrated that Fos and Jun proteins combine to form stable AP-1 heterodimers, which bind to AP-1 consensus sequences present in numerous genes associated with cell proliferative response and extracellular matrix production.	bind
35858	1	8404	5	13	NULL	NULL	NULL	angiopoietins	GP		bind					Tie2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_6_2179_s_13	10854238	5- 7  All known angiopoietins bind to Tie2, but it is still unclear as to whether they use the closely related receptor Tie1.	bind
28653	1	8404	6	NULL	NULL	0	NULL	angiopoietins	NULL		bind	NULL				Tie2	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_6_2179_s_13	10854238	5- 7  All known angiopoietins bind to Tie2, but it is still unclear as to whether they use the closely related receptor Tie1.	bind
35860	1	8407	5	13	NULL	NULL	NULL	5-Br-nosc	Chemical		bind					tubulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_63_4_799_s_111	12644580	5-Br-nosc and Rd 5-Br-nosc Have Higher Tubulin Binding Activity than Noscapine.	bind
35861	2	8407	5	13	NULL	NULL	NULL	Rd 5-Br-nosc	Chemical		bind					tubulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_63_4_799_s_111	12644580	5-Br-nosc and Rd 5-Br-nosc Have Higher Tubulin Binding Activity than Noscapine.	bind
35862	3	8407	5	13	NULL	NULL	NULL	noscapine	Chemical		bind					tubulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_63_4_799_s_111	12644580	5-Br-nosc and Rd 5-Br-nosc Have Higher Tubulin Binding Activity than Noscapine.	bind
35863	4	8407	5	13	NULL	NULL	NULL	statement 1	Process		higher affinity than					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_63_4_799_s_111	12644580	5-Br-nosc and Rd 5-Br-nosc Have Higher Tubulin Binding Activity than Noscapine.	bind
35864	5	8407	5	13	NULL	NULL	NULL	statement 2	Process		higher affinity than					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_63_4_799_s_111	12644580	5-Br-nosc and Rd 5-Br-nosc Have Higher Tubulin Binding Activity than Noscapine.	bind
28654	1	8407	6	NULL	NULL	0	NULL	5-Br-nosc	NULL		bind	NULL				tubulin	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_63_4_799_s_111	12644580	5-Br-nosc and Rd 5-Br-nosc Have Higher Tubulin Binding Activity than Noscapine.	bind
28655	2	8407	6	NULL	NULL	0	NULL	Rd 5-Br-nosc	NULL		bind	NULL				tubulin	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_63_4_799_s_111	12644580	5-Br-nosc and Rd 5-Br-nosc Have Higher Tubulin Binding Activity than Noscapine.	bind
28656	3	8407	6	NULL	NULL	0	NULL	noscapine	NULL		bind	NULL				tubulin	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_63_4_799_s_111	12644580	5-Br-nosc and Rd 5-Br-nosc Have Higher Tubulin Binding Activity than Noscapine.	bind
28669	4	8407	6	10	NULL	0	NULL	statement 1	NULL	affinity of	is higher than	NULL				statement 3	NULL	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_63_4_799_s_111	12644580	5-Br-nosc and Rd 5-Br-nosc Have Higher Tubulin Binding Activity than Noscapine.	bind
28670	5	8407	6	NULL	NULL	0	NULL	statement 2	NULL	affinity of	is higher than	NULL				statement 3	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_63_4_799_s_111	12644580	5-Br-nosc and Rd 5-Br-nosc Have Higher Tubulin Binding Activity than Noscapine.	bind
36736	1	8408	5	13	NULL	NULL	NULL	ephrin B1	GP		does not increase					JNK	GP	activity of			NULL	cells transfected with kinase defective (K652R) mutant receptors	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_3_1303_s_148	9430661	5-fold increases in JNK activity in cells transfected with either vector control (pSRalpha) or wild type EphB1 (pSRalpha-EphB1/HA). In contrast, ephrin B1 failed to increase JNK activity in cells transfected with either kinase defective (K652R) or Nck binding defective (Y594F) mutant receptors.	bind
36737	2	8408	5	13	NULL	NULL	NULL	ephrin B1	GP		does not increase					JNK	GP	activity of			NULL	cells transfected with Nck binding defective (Y594F) mutant receptors	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_3_1303_s_148	9430661	5-fold increases in JNK activity in cells transfected with either vector control (pSRalpha) or wild type EphB1 (pSRalpha-EphB1/HA). In contrast, ephrin B1 failed to increase JNK activity in cells transfected with either kinase defective (K652R) or Nck binding defective (Y594F) mutant receptors.	bind
28828	1	8408	6	10	NULL	0	NULL	ephrin B1	NULL		failed to increase	NULL				JNK	NULL	activity of			NULL	cells transfected with kinase defective (K652R) mutant receptors	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_3_1303_s_148	9430661	5-fold increases in JNK activity in cells transfected with either vector control (pSRalpha) or wild type EphB1 (pSRalpha-EphB1/HA). In contrast, ephrin B1 failed to increase JNK activity in cells transfected with either kinase defective (K652R) or Nck binding defective (Y594F) mutant receptors.	bind
28829	2	8408	6	10	NULL	0	NULL	ephrin B1	NULL		failed to increase	NULL				JNK	NULL	activity of			NULL	cells transfected with Nck binding defective (Y594F) mutant receptors	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_3_1303_s_148	9430661	5-fold increases in JNK activity in cells transfected with either vector control (pSRalpha) or wild type EphB1 (pSRalpha-EphB1/HA). In contrast, ephrin B1 failed to increase JNK activity in cells transfected with either kinase defective (K652R) or Nck binding defective (Y594F) mutant receptors.	bind
35865	1	8409	5	13	NULL	NULL	NULL	DnaA protein	GP		bind					oriC fragment	NucleicAcid	radiolabeled			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_37_23017_s_168	9287298	5-fold molar excess of unlabeled  oriC was required as a competitor to reduce to about 50% the binding of either DnaA protein or T435M to the radiolabeled  oriC fragment.	bind
35866	2	8409	5	13	NULL	NULL	NULL	T435M	GP		bind					oriC fragment	NucleicAcid	radiolabeled			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_37_23017_s_168	9287298	5-fold molar excess of unlabeled  oriC was required as a competitor to reduce to about 50% the binding of either DnaA protein or T435M to the radiolabeled  oriC fragment.	bind
35867	3	8409	5	13	NULL	NULL	NULL	oriC	NucleicAcid	unlabeled	bind					 oriC fragment	NucleicAcid	radiolabeled			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_37_23017_s_168	9287298	5-fold molar excess of unlabeled  oriC was required as a competitor to reduce to about 50% the binding of either DnaA protein or T435M to the radiolabeled  oriC fragment.	bind
35869	4	8409	5	13	NULL	NULL	NULL	statement 1	Process		competes with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_37_23017_s_168	9287298	5-fold molar excess of unlabeled  oriC was required as a competitor to reduce to about 50% the binding of either DnaA protein or T435M to the radiolabeled  oriC fragment.	bind
35870	6	8409	5	13	NULL	NULL	NULL	statement 3	Process		reduces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_37_23017_s_168	9287298	5-fold molar excess of unlabeled  oriC was required as a competitor to reduce to about 50% the binding of either DnaA protein or T435M to the radiolabeled  oriC fragment.	bind
35871	5	8409	5	13	NULL	NULL	NULL	statement 2	Process		competes with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_37_23017_s_168	9287298	5-fold molar excess of unlabeled  oriC was required as a competitor to reduce to about 50% the binding of either DnaA protein or T435M to the radiolabeled  oriC fragment.	bind
35872	7	8409	5	13	NULL	NULL	NULL	statement 3	Process		reduces					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_37_23017_s_168	9287298	5-fold molar excess of unlabeled  oriC was required as a competitor to reduce to about 50% the binding of either DnaA protein or T435M to the radiolabeled  oriC fragment.	bind
28830	1	8409	6	NULL	NULL	0	NULL	DnaA protein	NULL		bind	NULL				oriC fragment	NULL	radiolabeled			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_37_23017_s_168	9287298	5-fold molar excess of unlabeled  oriC was required as a competitor to reduce to about 50% the binding of either DnaA protein or T435M to the radiolabeled  oriC fragment.	bind
28831	2	8409	6	NULL	NULL	0	NULL		NULL		bind	NULL		T435M		oriC fragment	NULL	radiolabeled			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_37_23017_s_168	9287298	5-fold molar excess of unlabeled  oriC was required as a competitor to reduce to about 50% the binding of either DnaA protein or T435M to the radiolabeled  oriC fragment.	bind
28832	3	8409	6	NULL	NULL	0	NULL	oriC	NULL	unlabeled	bind	NULL				oriC fragment	NULL	radiolabeled			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_37_23017_s_168	9287298	5-fold molar excess of unlabeled  oriC was required as a competitor to reduce to about 50% the binding of either DnaA protein or T435M to the radiolabeled  oriC fragment.	bind
28833	4	8409	6	NULL	NULL	0	NULL	statement 1	NULL		competes	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_37_23017_s_168	9287298	5-fold molar excess of unlabeled  oriC was required as a competitor to reduce to about 50% the binding of either DnaA protein or T435M to the radiolabeled  oriC fragment.	bind
28834	5	8409	6	NULL	NULL	0	NULL	statement 2	NULL		competes	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_37_23017_s_168	9287298	5-fold molar excess of unlabeled  oriC was required as a competitor to reduce to about 50% the binding of either DnaA protein or T435M to the radiolabeled  oriC fragment.	bind
35873	1	8410	5	13	NULL	NULL	NULL	1,25(OH)2D3-receptor complex	GP	intestinal;;cytosolic	bind					DNA	NucleicAcid	heterologous			NULL		NULL	NULL	NULL	NULL	abs-batch0760-0779_biull-eksp-biol-med_106_12_2850038_s_3	2850038	5-fold)  increase of intestinal cytosolic 1,25(OH)2D3-receptor complex binding  with heterologous DNA, whereas maximum binding capacity and equilibrium  dissociation constant of cytosolic 1,25 (OH)2D3 receptors did not change.	bind
28835	1	8410	6	10	NULL	0	NULL	1,25(OH)2D3-receptor complex		intestinal;; cytosolic	bind					DNA		heterologous			NULL		NULL	NULL	NULL	NULL	abs-batch0760-0779_biull-eksp-biol-med_106_12_2850038_s_3	2850038	5-fold)  increase of intestinal cytosolic 1,25(OH)2D3-receptor complex binding  with heterologous DNA, whereas maximum binding capacity and equilibrium  dissociation constant of cytosolic 1,25 (OH)2D3 receptors did not change.	bind
35876	1	8411	5	13	NULL	NULL	NULL	5-HT1A receptor	GP		bind					G proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_135_5_1115_s_6	11877317	5-HT1A receptor binding and coupling to G proteins were assessed using [3]-8-OH-DPAT and [35]-GTPgammaS autoradiography, respectively.	bind
35878	2	8411	5	13	NULL	NULL	NULL	5-HT1A receptor	GP		couple to					G proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_135_5_1115_s_6	11877317	5-HT1A receptor binding and coupling to G proteins were assessed using [3]-8-OH-DPAT and [35]-GTPgammaS autoradiography, respectively.	bind
28836	1	8411	6	NULL	NULL	0	NULL	HT1A receptor	NULL		bind	NULL				G proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_5_1115_s_6	11877317	5-HT1A receptor binding and coupling to G proteins were assessed using [3]-8-OH-DPAT and [35]-GTPgammaS autoradiography, respectively.	bind
28837	2	8411	6	NULL	NULL	0	NULL	HT1A receptor	NULL		couples to	NULL				G proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_5_1115_s_6	11877317	5-HT1A receptor binding and coupling to G proteins were assessed using [3]-8-OH-DPAT and [35]-GTPgammaS autoradiography, respectively.	bind
35880	1	8412	5	13	NULL	NULL	NULL	5-HT2A receptor	GP		bind					VMAT2	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainres_835_2_104_s_62	10415365	5-HT2A receptor and vesicular monoamine transporter (VMAT2) binding ( Kd and  Bmax) were measured by [3]ketanserin (DuPont, specific activity 85.1 Ci/mmol) and [125]TBZ (synthesized by Dr. M.-P. Kung, specific activity 2200 Ci/mmol) using saturation assays.	bind
35882	2	8412	5	13	NULL	NULL	NULL	VMAT2	GP		is					vesicular monoamine transporter	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainres_835_2_104_s_62	10415365	5-HT2A receptor and vesicular monoamine transporter (VMAT2) binding ( Kd and  Bmax) were measured by [3]ketanserin (DuPont, specific activity 85.1 Ci/mmol) and [125]TBZ (synthesized by Dr. M.-P. Kung, specific activity 2200 Ci/mmol) using saturation assays.	bind
28838	1	8412	6	NULL	NULL	0	NULL	VMAT	NULL		is	NULL				vesicular monoamine transporter	NULL				NULL		0	NULL	NULL	NULL	gw60_brainres_835_2_104_s_62	10415365	5-HT2A receptor and vesicular monoamine transporter (VMAT2) binding ( Kd and  Bmax) were measured by [3]ketanserin (DuPont, specific activity 85.1 Ci/mmol) and [125]TBZ (synthesized by Dr. M.-P. Kung, specific activity 2200 Ci/mmol) using saturation assays.	bind
28839	2	8412	6	NULL	NULL	0	NULL	HT2A receptor	NULL		bind	NULL				VMAT2	NULL				NULL		0	NULL	NULL	NULL	gw60_brainres_835_2_104_s_62	10415365	5-HT2A receptor and vesicular monoamine transporter (VMAT2) binding ( Kd and  Bmax) were measured by [3]ketanserin (DuPont, specific activity 85.1 Ci/mmol) and [125]TBZ (synthesized by Dr. M.-P. Kung, specific activity 2200 Ci/mmol) using saturation assays.	bind
35883	1	8413	5	13	NULL	NULL	NULL	Rho GTPase	GP	stimulation of	activates					SRF	GP				NULL		NULL	NULL	NULL	NULL	gw70_jneurosci_25_34_7821_s_309	16120784	5-HT7R/12 signaling and regulation of gene transcription   One of the physiological consequences of Rho GTPase stimulation is the activation of a transcription factor, SRF, which binds to the SRE.	bind
35884	2	8413	5	13	NULL	NULL	NULL	SRF	GP		bind									SRE	NULL		NULL	NULL	NULL	NULL	gw70_jneurosci_25_34_7821_s_309	16120784	5-HT7R/12 signaling and regulation of gene transcription   One of the physiological consequences of Rho GTPase stimulation is the activation of a transcription factor, SRF, which binds to the SRE.	bind
35885	3	8413	5	13	NULL	NULL	NULL	SRF	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_jneurosci_25_34_7821_s_309	16120784	5-HT7R/12 signaling and regulation of gene transcription   One of the physiological consequences of Rho GTPase stimulation is the activation of a transcription factor, SRF, which binds to the SRE.	bind
28840	1	8413	6	NULL	NULL	0	NULL	SRF	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw70_jneurosci_25_34_7821_s_309	16120784	5-HT7R/12 signaling and regulation of gene transcription   One of the physiological consequences of Rho GTPase stimulation is the activation of a transcription factor, SRF, which binds to the SRE.	bind
28841	2	8413	6	NULL	NULL	0	NULL	rho GTPase	NULL	stimulation of	leads to	NULL				SRF	NULL	activation of			NULL		0	NULL	NULL	NULL	gw70_jneurosci_25_34_7821_s_309	16120784	5-HT7R/12 signaling and regulation of gene transcription   One of the physiological consequences of Rho GTPase stimulation is the activation of a transcription factor, SRF, which binds to the SRE.	bind
28842	3	8413	6	NULL	NULL	0	NULL	SRF	NULL		bind	NULL					NULL			SRE	NULL		0	NULL	NULL	NULL	gw70_jneurosci_25_34_7821_s_309	16120784	5-HT7R/12 signaling and regulation of gene transcription   One of the physiological consequences of Rho GTPase stimulation is the activation of a transcription factor, SRF, which binds to the SRE.	bind
35886	1	8414	5	13	NULL	NULL	NULL	5-Lipoxygenase	GP		does not bind					GTPase-activating protein	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_269_39_7929073_s_7	7929073	5-Lipoxygenase did not bind to the SH3 domains of other  signaling proteins, such as GTPase-activating protein and phospholipase  C gamma; however, it bound to certain cytoskeletal proteins including  alpha-actinin and actin.	bind
35888	2	8414	5	13	NULL	NULL	NULL	5-Lipoxygenase	GP		does not bind					phospholipase C gamma	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_269_39_7929073_s_7	7929073	5-Lipoxygenase did not bind to the SH3 domains of other  signaling proteins, such as GTPase-activating protein and phospholipase  C gamma; however, it bound to certain cytoskeletal proteins including  alpha-actinin and actin.	bind
35890	3	8414	5	13	NULL	NULL	NULL	5-Lipoxygenase	GP		bind					alpha-actinin	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_269_39_7929073_s_7	7929073	5-Lipoxygenase did not bind to the SH3 domains of other  signaling proteins, such as GTPase-activating protein and phospholipase  C gamma; however, it bound to certain cytoskeletal proteins including  alpha-actinin and actin.	bind
35892	4	8414	5	13	NULL	NULL	NULL	5-Lipoxygenase	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_269_39_7929073_s_7	7929073	5-Lipoxygenase did not bind to the SH3 domains of other  signaling proteins, such as GTPase-activating protein and phospholipase  C gamma; however, it bound to certain cytoskeletal proteins including  alpha-actinin and actin.	bind
35893	5	8414	5	13	NULL	NULL	NULL	alpha-actinin	GP		is a type of					cytoskeletal proteins	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_269_39_7929073_s_7	7929073	5-Lipoxygenase did not bind to the SH3 domains of other  signaling proteins, such as GTPase-activating protein and phospholipase  C gamma; however, it bound to certain cytoskeletal proteins including  alpha-actinin and actin.	bind
35894	6	8414	5	13	NULL	NULL	NULL	actin	GP		is a type of					cytoskeletal proteins	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_269_39_7929073_s_7	7929073	5-Lipoxygenase did not bind to the SH3 domains of other  signaling proteins, such as GTPase-activating protein and phospholipase  C gamma; however, it bound to certain cytoskeletal proteins including  alpha-actinin and actin.	bind
35897	7	8414	5	13	NULL	NULL	NULL	GTPase-activating protein	GP		is a type of					signaling proteins	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_269_39_7929073_s_7	7929073	5-Lipoxygenase did not bind to the SH3 domains of other  signaling proteins, such as GTPase-activating protein and phospholipase  C gamma; however, it bound to certain cytoskeletal proteins including  alpha-actinin and actin.	bind
35898	8	8414	5	13	NULL	NULL	NULL	phospholipase C gamma	GP		is a type of					signaling proteins	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_269_39_7929073_s_7	7929073	5-Lipoxygenase did not bind to the SH3 domains of other  signaling proteins, such as GTPase-activating protein and phospholipase  C gamma; however, it bound to certain cytoskeletal proteins including  alpha-actinin and actin.	bind
28843	1	8414	6	NULL	NULL	0	NULL	GTPase-activating protein	NULL		is a type of	NULL				signaling protein	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_269_39_7929073_s_7	7929073	5-Lipoxygenase did not bind to the SH3 domains of other  signaling proteins, such as GTPase-activating protein and phospholipase  C gamma; however, it bound to certain cytoskeletal proteins including  alpha-actinin and actin.	bind
28844	2	8414	6	NULL	NULL	0	NULL	phospholipase C gamma	NULL		is a type of	NULL				signaling protein	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_269_39_7929073_s_7	7929073	5-Lipoxygenase did not bind to the SH3 domains of other  signaling proteins, such as GTPase-activating protein and phospholipase  C gamma; however, it bound to certain cytoskeletal proteins including  alpha-actinin and actin.	bind
28846	3	8414	6	NULL	NULL	0	NULL	alpha-actinin	NULL		is a type of	NULL				cytoskeletal protein	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_269_39_7929073_s_7	7929073	5-Lipoxygenase did not bind to the SH3 domains of other  signaling proteins, such as GTPase-activating protein and phospholipase  C gamma; however, it bound to certain cytoskeletal proteins including  alpha-actinin and actin.	bind
28847	4	8414	6	NULL	NULL	0	NULL	actin	NULL		is a type of	NULL				cytoskeletal protein	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_269_39_7929073_s_7	7929073	5-Lipoxygenase did not bind to the SH3 domains of other  signaling proteins, such as GTPase-activating protein and phospholipase  C gamma; however, it bound to certain cytoskeletal proteins including  alpha-actinin and actin.	bind
28848	5	8414	6	NULL	NULL	0	NULL	5-Lipoxygenase	NULL		does not bind	NULL				GTPase-activating protein	NULL		SH3 domain		NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_269_39_7929073_s_7	7929073	5-Lipoxygenase did not bind to the SH3 domains of other  signaling proteins, such as GTPase-activating protein and phospholipase  C gamma; however, it bound to certain cytoskeletal proteins including  alpha-actinin and actin.	bind
28849	6	8414	6	NULL	NULL	0	NULL	5-Lipoxygenase	NULL		does not bind	NULL				phospholipase C gamma	NULL		SH3 domain		NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_269_39_7929073_s_7	7929073	5-Lipoxygenase did not bind to the SH3 domains of other  signaling proteins, such as GTPase-activating protein and phospholipase  C gamma; however, it bound to certain cytoskeletal proteins including  alpha-actinin and actin.	bind
28850	7	8414	6	NULL	NULL	0	NULL	5-Lipoxygenase	NULL		bind	NULL				alpha-actinin	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_269_39_7929073_s_7	7929073	5-Lipoxygenase did not bind to the SH3 domains of other  signaling proteins, such as GTPase-activating protein and phospholipase  C gamma; however, it bound to certain cytoskeletal proteins including  alpha-actinin and actin.	bind
28851	8	8414	6	NULL	NULL	0	NULL	5-Lipoxygenase	NULL		bind	NULL				actin	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_269_39_7929073_s_7	7929073	5-Lipoxygenase did not bind to the SH3 domains of other  signaling proteins, such as GTPase-activating protein and phospholipase  C gamma; however, it bound to certain cytoskeletal proteins including  alpha-actinin and actin.	bind
35900	1	8415	5	13	NULL	NULL	NULL	Histone H1	GP		bind		preferentially			superhelical DNA molecules	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_19_4043_s_480	11574687	50       Ivanchenko,M., Zlatanova,J. and van Holde,K. (1997) Histone H1 preferentially binds to superhelical DNA molecules of higher compaction.	bind
28852	1	8415	6	NULL	NULL	0	NULL	Histone H1	NULL		bind	NULL	preferentially			superhelical DNA molecules	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_19_4043_s_480	11574687	50       Ivanchenko,M., Zlatanova,J. and van Holde,K. (1997) Histone H1 preferentially binds to superhelical DNA molecules of higher compaction.	bind
35902	2	8419	5	13	NULL	NULL	NULL	statement 1	GP		bind					GST-p38alpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_6905_s_103	11238443	50 mug of thrombin-digested GST-ERK1 was added to GST-p38alpha beads, and ERK1 that bound to p38 was detected by Western blotting with anti-ERK1-CT antibody.	bind
47874	1	8419	5	13	NULL	NULL	NULL	GST-ERK1 	GP		digested with					thrombin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_6905_s_103	11238443	50 mug of thrombin-digested GST-ERK1 was added to GST-p38alpha beads, and ERK1 that bound to p38 was detected by Western blotting with anti-ERK1-CT antibody.	bind
28853	2	8419	6	10	NULL	0	NULL	statement 1	NULL		bind	NULL				p38	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_6905_s_103	11238443	50 mug of thrombin-digested GST-ERK1 was added to GST-p38alpha beads, and ERK1 that bound to p38 was detected by Western blotting with anti-ERK1-CT antibody.	bind
47875	1	8419	6	10	NULL	0	NULL	GST-ERK1 	NULL		digested with	NULL				thrombin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_10_6905_s_103	11238443	50 mug of thrombin-digested GST-ERK1 was added to GST-p38alpha beads, and ERK1 that bound to p38 was detected by Western blotting with anti-ERK1-CT antibody.	bind
35903	1	8424	5	13	NULL	NULL	NULL	OKA	Chemical		induce					NF-kappaB	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_28_25804_s_193	11320078	50 nM OKA was able to both induce NF-kappaB binding (Fig.  4 A, lane 18) and block the effects of TPA (Fig.  4 A, lane 12) on the mobility of the pets complex.	bind
35904	2	8424	5	13	NULL	NULL	NULL	TPA	Chemical		effect					pets complex	GP	mobility of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_28_25804_s_193	11320078	50 nM OKA was able to both induce NF-kappaB binding (Fig.  4 A, lane 18) and block the effects of TPA (Fig.  4 A, lane 12) on the mobility of the pets complex.	bind
35905	3	8424	5	13	NULL	NULL	NULL	OKA	Chemical		block					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_28_25804_s_193	11320078	50 nM OKA was able to both induce NF-kappaB binding (Fig.  4 A, lane 18) and block the effects of TPA (Fig.  4 A, lane 12) on the mobility of the pets complex.	bind
28854	1	8424	6	NULL	NULL	0	NULL	OKA	NULL		induce	NULL				NF-kappaB	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_28_25804_s_193	11320078	50 nM OKA was able to both induce NF-kappaB binding (Fig.  4 A, lane 18) and block the effects of TPA (Fig.  4 A, lane 12) on the mobility of the pets complex.	bind
28855	2	8424	6	NULL	NULL	0	NULL	TPA	NULL		effects	NULL				pets complex	NULL	mobility of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_28_25804_s_193	11320078	50 nM OKA was able to both induce NF-kappaB binding (Fig.  4 A, lane 18) and block the effects of TPA (Fig.  4 A, lane 12) on the mobility of the pets complex.	bind
28856	3	8424	6	NULL	NULL	0	NULL	OKA	NULL		block	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_28_25804_s_193	11320078	50 nM OKA was able to both induce NF-kappaB binding (Fig.  4 A, lane 18) and block the effects of TPA (Fig.  4 A, lane 12) on the mobility of the pets complex.	bind
35906	1	8425	5	13	NULL	NULL	NULL	VEGF	GP		bind					KDR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_32_20556_s_341	9685413	50% inhibition of VEGF binding to KDR required about 2 or 3 x 10 12M for aptamers t22-OMe and t44-OMe, respectively, 6 x 10 11M for t2-OMe, and 5 x 10 8M for scr-t44-OMe.	bind
35907	2	8425	5	13	NULL	NULL	NULL	t22-OMe	NucleicAcid		is a type of					aptamer	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_32_20556_s_341	9685413	50% inhibition of VEGF binding to KDR required about 2 or 3 x 10 12M for aptamers t22-OMe and t44-OMe, respectively, 6 x 10 11M for t2-OMe, and 5 x 10 8M for scr-t44-OMe.	bind
35908	3	8425	5	13	NULL	NULL	NULL	t44-OMe	NucleicAcid		is a type of					aptamer	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_32_20556_s_341	9685413	50% inhibition of VEGF binding to KDR required about 2 or 3 x 10 12M for aptamers t22-OMe and t44-OMe, respectively, 6 x 10 11M for t2-OMe, and 5 x 10 8M for scr-t44-OMe.	bind
35909	4	8425	5	13	NULL	NULL	NULL	t22-OMe	NucleicAcid		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_32_20556_s_341	9685413	50% inhibition of VEGF binding to KDR required about 2 or 3 x 10 12M for aptamers t22-OMe and t44-OMe, respectively, 6 x 10 11M for t2-OMe, and 5 x 10 8M for scr-t44-OMe.	bind
35910	5	8425	5	13	NULL	NULL	NULL	t44-OMe	NucleicAcid		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_32_20556_s_341	9685413	50% inhibition of VEGF binding to KDR required about 2 or 3 x 10 12M for aptamers t22-OMe and t44-OMe, respectively, 6 x 10 11M for t2-OMe, and 5 x 10 8M for scr-t44-OMe.	bind
28857	1	8425	6	NULL	NULL	0	NULL	VEGF	NULL		bind	NULL				KDR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_32_20556_s_341	9685413	50% inhibition of VEGF binding to KDR required about 2 or 3 x 10 12M for aptamers t22-OMe and t44-OMe, respectively, 6 x 10 11M for t2-OMe, and 5 x 10 8M for scr-t44-OMe.	bind
48139	2	8425	6	10	NULL	0	NULL	t22-OMe	NULL		is a type of	NULL				aptamer	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_32_20556_s_341	9685413	50% inhibition of VEGF binding to KDR required about 2 or 3 x 10 12M for aptamers t22-OMe and t44-OMe, respectively, 6 x 10 11M for t2-OMe, and 5 x 10 8M for scr-t44-OMe.	bind
48140	3	8425	6	10	NULL	0	NULL	t44-OMe	NULL		is a type of	NULL				aptamer	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_32_20556_s_341	9685413	50% inhibition of VEGF binding to KDR required about 2 or 3 x 10 12M for aptamers t22-OMe and t44-OMe, respectively, 6 x 10 11M for t2-OMe, and 5 x 10 8M for scr-t44-OMe.	bind
48141	4	8425	6	10	NULL	0	NULL	t22-OMe	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_32_20556_s_341	9685413	50% inhibition of VEGF binding to KDR required about 2 or 3 x 10 12M for aptamers t22-OMe and t44-OMe, respectively, 6 x 10 11M for t2-OMe, and 5 x 10 8M for scr-t44-OMe.	bind
48142	5	8425	6	10	NULL	0	NULL	t44-OMe	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_32_20556_s_341	9685413	50% inhibition of VEGF binding to KDR required about 2 or 3 x 10 12M for aptamers t22-OMe and t44-OMe, respectively, 6 x 10 11M for t2-OMe, and 5 x 10 8M for scr-t44-OMe.	bind
35911	1	8426	5	13	NULL	NULL	NULL	pRB	GP		associate with		specifically			E2F-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_3_919_s_275	10980131	50, 55- 61 pRB seems to associate specifically with E2F-1, E2F-2, and E2F-3, 59 whereas p107 binds E2F-4 56, 61  and p130 binds E2F-4 and E2F-5.	bind
35913	2	8426	5	13	NULL	NULL	NULL	pRB	GP		associate with		specifically			E2F-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_3_919_s_275	10980131	50, 55- 61 pRB seems to associate specifically with E2F-1, E2F-2, and E2F-3, 59 whereas p107 binds E2F-4 56, 61  and p130 binds E2F-4 and E2F-5.	bind
35914	3	8426	5	13	NULL	NULL	NULL	pRB	GP		associate with		specifically			E2F-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_3_919_s_275	10980131	50, 55- 61 pRB seems to associate specifically with E2F-1, E2F-2, and E2F-3, 59 whereas p107 binds E2F-4 56, 61  and p130 binds E2F-4 and E2F-5.	bind
35915	4	8426	5	13	NULL	NULL	NULL	p107	GP		bind					E2F-4	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_3_919_s_275	10980131	50, 55- 61 pRB seems to associate specifically with E2F-1, E2F-2, and E2F-3, 59 whereas p107 binds E2F-4 56, 61  and p130 binds E2F-4 and E2F-5.	bind
35916	5	8426	5	13	NULL	NULL	NULL	p130	GP		bind					E2F-4	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_3_919_s_275	10980131	50, 55- 61 pRB seems to associate specifically with E2F-1, E2F-2, and E2F-3, 59 whereas p107 binds E2F-4 56, 61  and p130 binds E2F-4 and E2F-5.	bind
35917	6	8426	5	13	NULL	NULL	NULL	p130	GP		bind					E2F-5	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_3_919_s_275	10980131	50, 55- 61 pRB seems to associate specifically with E2F-1, E2F-2, and E2F-3, 59 whereas p107 binds E2F-4 56, 61  and p130 binds E2F-4 and E2F-5.	bind
28858	1	8426	6	NULL	NULL	0	NULL	pRB	NULL		associate	NULL	specifically			E2F-1	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_3_919_s_275	10980131	50, 55- 61 pRB seems to associate specifically with E2F-1, E2F-2, and E2F-3, 59 whereas p107 binds E2F-4 56, 61  and p130 binds E2F-4 and E2F-5.	bind
28859	2	8426	6	NULL	NULL	0	NULL	pRB	NULL		associate	NULL	specifically			E2F-2	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_3_919_s_275	10980131	50, 55- 61 pRB seems to associate specifically with E2F-1, E2F-2, and E2F-3, 59 whereas p107 binds E2F-4 56, 61  and p130 binds E2F-4 and E2F-5.	bind
28860	3	8426	6	NULL	NULL	0	NULL	pRB	NULL		associate	NULL	specifically			E2F-3	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_3_919_s_275	10980131	50, 55- 61 pRB seems to associate specifically with E2F-1, E2F-2, and E2F-3, 59 whereas p107 binds E2F-4 56, 61  and p130 binds E2F-4 and E2F-5.	bind
28861	4	8426	6	NULL	NULL	0	NULL	p107	NULL		bind	NULL				E2F-4	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_3_919_s_275	10980131	50, 55- 61 pRB seems to associate specifically with E2F-1, E2F-2, and E2F-3, 59 whereas p107 binds E2F-4 56, 61  and p130 binds E2F-4 and E2F-5.	bind
28862	5	8426	6	NULL	NULL	0	NULL	p130	NULL		bind	NULL				E2F-4	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_3_919_s_275	10980131	50, 55- 61 pRB seems to associate specifically with E2F-1, E2F-2, and E2F-3, 59 whereas p107 binds E2F-4 56, 61  and p130 binds E2F-4 and E2F-5.	bind
28863	6	8426	6	NULL	NULL	0	NULL	p130	NULL		bind	NULL				E2F-5	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_3_919_s_275	10980131	50, 55- 61 pRB seems to associate specifically with E2F-1, E2F-2, and E2F-3, 59 whereas p107 binds E2F-4 56, 61  and p130 binds E2F-4 and E2F-5.	bind
36086	1	8427	5	13	NULL	NULL	NULL	Pit-1	GP		enhance					Pitx2 bound complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_32_20066_s_195	9685346	50-fold molar excess of unlabeled  bicoid competitor DNA competed for the Pit-1-enhanced Pitx2 bound complex.	bind
36104	2	8427	5	13	NULL	NULL	NULL	bicoid DNA	NucleicAcid	unlabeled	bind					Pitx2 bound complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_32_20066_s_195	9685346	50-fold molar excess of unlabeled  bicoid competitor DNA competed for the Pit-1-enhanced Pitx2 bound complex.	bind
36105	3	8427	5	13	NULL	NULL	NULL	statement 2	Process		competes with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_32_20066_s_195	9685346	50-fold molar excess of unlabeled  bicoid competitor DNA competed for the Pit-1-enhanced Pitx2 bound complex.	bind
28864	1	8427	6	NULL	NULL	0	NULL	Pit-1	NULL		enhances	NULL				Pitx2 bound complex	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_32_20066_s_195	9685346	50-fold molar excess of unlabeled  bicoid competitor DNA competed for the Pit-1-enhanced Pitx2 bound complex.	bind
29029	2	8427	6	NULL	NULL	0	NULL	bicoid competitor DNA	NULL	unlabeled	competes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_32_20066_s_195	9685346	50-fold molar excess of unlabeled  bicoid competitor DNA competed for the Pit-1-enhanced Pitx2 bound complex.	bind
47876	3	8427	6	10	NULL	0	NULL	statement 2	NULL		compete with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_32_20066_s_195	9685346	50-fold molar excess of unlabeled  bicoid competitor DNA competed for the Pit-1-enhanced Pitx2 bound complex.	bind
36106	1	8435	5	13	NULL	NULL	NULL	PDGF-AA	GP		does not supress					SMC	Cell	migration of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_3_305_s_239	9710123	51  Our data that PDGF-AA failed to suppress SMC migration on a Vitrogen-coated filter are consistent with the report that HSPG binds to intact fibrillar type I collagen but not to pepsin-digested type I collagen, such as Vitrogen.	bind
36107	2	8435	5	13	NULL	NULL	NULL	HSPG	GP		bind					fibrillar type I collagen	GP	intact			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_3_305_s_239	9710123	51  Our data that PDGF-AA failed to suppress SMC migration on a Vitrogen-coated filter are consistent with the report that HSPG binds to intact fibrillar type I collagen but not to pepsin-digested type I collagen, such as Vitrogen.	bind
36108	3	8435	5	13	NULL	NULL	NULL	HSPG	GP		does not bind					Vitrogen	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_3_305_s_239	9710123	51  Our data that PDGF-AA failed to suppress SMC migration on a Vitrogen-coated filter are consistent with the report that HSPG binds to intact fibrillar type I collagen but not to pepsin-digested type I collagen, such as Vitrogen.	bind
36109	4	8435	5	13	NULL	NULL	NULL	Vitrogen	GP		is a type of					pepsin-digested type I collagen	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_3_305_s_239	9710123	51  Our data that PDGF-AA failed to suppress SMC migration on a Vitrogen-coated filter are consistent with the report that HSPG binds to intact fibrillar type I collagen but not to pepsin-digested type I collagen, such as Vitrogen.	bind
28865	1	8435	6	10	NULL	0	NULL	vitrogen			is a type of					pepsin-digested type I collagen					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_3_305_s_239	9710123	51  Our data that PDGF-AA failed to suppress SMC migration on a Vitrogen-coated filter are consistent with the report that HSPG binds to intact fibrillar type I collagen but not to pepsin-digested type I collagen, such as Vitrogen.	bind
28866	2	8435	6	NULL	NULL	0	NULL	HSPG	NULL		bind	NULL				fibrillar type I collagen	NULL	intact			NULL		0	NULL	NULL	NULL	gw60_circulationres_83_3_305_s_239	9710123	51  Our data that PDGF-AA failed to suppress SMC migration on a Vitrogen-coated filter are consistent with the report that HSPG binds to intact fibrillar type I collagen but not to pepsin-digested type I collagen, such as Vitrogen.	bind
28867	3	8435	6	NULL	NULL	0	NULL	HSPG	NULL		does not bind	NULL				vitrogen	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_3_305_s_239	9710123	51  Our data that PDGF-AA failed to suppress SMC migration on a Vitrogen-coated filter are consistent with the report that HSPG binds to intact fibrillar type I collagen but not to pepsin-digested type I collagen, such as Vitrogen.	bind
28868	4	8435	6	NULL	NULL	0	NULL	PDGF-AA	NULL		failed to suppress	NULL				SMC	NULL	migration of			NULL		0	NULL	NULL	NULL	gw60_circulationres_83_3_305_s_239	9710123	51  Our data that PDGF-AA failed to suppress SMC migration on a Vitrogen-coated filter are consistent with the report that HSPG binds to intact fibrillar type I collagen but not to pepsin-digested type I collagen, such as Vitrogen.	bind
36110	1	8436	5	13	NULL	NULL	NULL	serum response factors	GP		bind									SRE	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_7_804_s_284	10205148	51  SRE is regulated by the binding of serum response factors and TCF, the transcriptional activities of which are enhanced by their phosphorylation.	bind
36111	2	8436	5	13	NULL	NULL	NULL	statement 1	Process		regulates									SRE	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_7_804_s_284	10205148	51  SRE is regulated by the binding of serum response factors and TCF, the transcriptional activities of which are enhanced by their phosphorylation.	bind
36112	3	8436	5	13	NULL	NULL	NULL	TCF	GP		bind									SRE	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_7_804_s_284	10205148	51  SRE is regulated by the binding of serum response factors and TCF, the transcriptional activities of which are enhanced by their phosphorylation.	bind
36113	4	8436	5	13	NULL	NULL	NULL	statement 3	Process		regulates									SRE	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_7_804_s_284	10205148	51  SRE is regulated by the binding of serum response factors and TCF, the transcriptional activities of which are enhanced by their phosphorylation.	bind
36114	5	8436	5	13	NULL	NULL	NULL	TCF	GP	phosphorylation of	enhance					TCF	GP	transcriptional activities of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_7_804_s_284	10205148	51  SRE is regulated by the binding of serum response factors and TCF, the transcriptional activities of which are enhanced by their phosphorylation.	bind
36115	6	8436	5	13	NULL	NULL	NULL	serum response factors	GP	phosphorylation of	enhance					serum response factors	GP	transcriptional activities of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_7_804_s_284	10205148	51  SRE is regulated by the binding of serum response factors and TCF, the transcriptional activities of which are enhanced by their phosphorylation.	bind
28869	1	8436	6	10	NULL	0	NULL	serum response factors	NULL		bind	NULL					NULL			SRE	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_7_804_s_284	10205148	51  SRE is regulated by the binding of serum response factors and TCF, the transcriptional activities of which are enhanced by their phosphorylation.	bind
28870	2	8436	6	NULL	NULL	0	NULL	statement 1	NULL		regulates	NULL					NULL			SRE	NULL		0	NULL	NULL	NULL	gw60_circulationres_84_7_804_s_284	10205148	51  SRE is regulated by the binding of serum response factors and TCF, the transcriptional activities of which are enhanced by their phosphorylation.	bind
28871	3	8436	6	NULL	NULL	0	NULL	serum response factors	NULL	phosphorylation of	enhances	NULL				serum response factor	NULL	transcriptional activity of			NULL		0	NULL	NULL	NULL	gw60_circulationres_84_7_804_s_284	10205148	51  SRE is regulated by the binding of serum response factors and TCF, the transcriptional activities of which are enhanced by their phosphorylation.	bind
28872	4	8436	6	NULL	NULL	0	NULL	TCF	NULL	phosphorylation of	enhances	NULL				TCF	NULL	transcriptional activity of			NULL		0	NULL	NULL	NULL	gw60_circulationres_84_7_804_s_284	10205148	51  SRE is regulated by the binding of serum response factors and TCF, the transcriptional activities of which are enhanced by their phosphorylation.	bind
48143	5	8436	6	10	NULL	0	NULL	TCF	NULL		bind	NULL					NULL			SRE	NULL		0	NULL	NULL	NULL	gw60_circulationres_84_7_804_s_284	10205148	51  SRE is regulated by the binding of serum response factors and TCF, the transcriptional activities of which are enhanced by their phosphorylation.	bind
48144	6	8436	6	10	NULL	0	NULL	statement 5	NULL		regulates	NULL					NULL			SRE	NULL		0	NULL	NULL	NULL	gw60_circulationres_84_7_804_s_284	10205148	51  SRE is regulated by the binding of serum response factors and TCF, the transcriptional activities of which are enhanced by their phosphorylation.	bind
36116	1	8437	5	13	NULL	NULL	NULL	cdk4	GP		complex with		stably			p16Ink4a	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_2_405_s_177	12163365	51, 52  Moreover, stable complexes between cdk4 and p16Ink4a were detected in several cell types and induction of these binary complexes caused marked inhibition of cdk2 activity by redistribution of cyclin and CKI subunits, particularly those involving p27Kip1 that bind and inhibit cdk2 activity.	bind
36117	2	8437	5	13	NULL	NULL	NULL	cdk4-p16Ink4a cpmplex	GP	induction of	inhibit					cdk2	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_2_405_s_177	12163365	51, 52  Moreover, stable complexes between cdk4 and p16Ink4a were detected in several cell types and induction of these binary complexes caused marked inhibition of cdk2 activity by redistribution of cyclin and CKI subunits, particularly those involving p27Kip1 that bind and inhibit cdk2 activity.	bind
36118	3	8437	5	13	NULL	NULL	NULL	cyclin subunits	GP	redistribution of 	leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_2_405_s_177	12163365	51, 52  Moreover, stable complexes between cdk4 and p16Ink4a were detected in several cell types and induction of these binary complexes caused marked inhibition of cdk2 activity by redistribution of cyclin and CKI subunits, particularly those involving p27Kip1 that bind and inhibit cdk2 activity.	bind
36119	4	8437	5	13	NULL	NULL	NULL	CKI subunits	GP	redistribution of	leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_2_405_s_177	12163365	51, 52  Moreover, stable complexes between cdk4 and p16Ink4a were detected in several cell types and induction of these binary complexes caused marked inhibition of cdk2 activity by redistribution of cyclin and CKI subunits, particularly those involving p27Kip1 that bind and inhibit cdk2 activity.	bind
36120	5	8437	5	13	NULL	NULL	NULL	p27Kip1	GP		bind					cdk2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_2_405_s_177	12163365	51, 52  Moreover, stable complexes between cdk4 and p16Ink4a were detected in several cell types and induction of these binary complexes caused marked inhibition of cdk2 activity by redistribution of cyclin and CKI subunits, particularly those involving p27Kip1 that bind and inhibit cdk2 activity.	bind
36121	6	8437	5	13	NULL	NULL	NULL	statement 5	Process		inhibit					cdk2	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_2_405_s_177	12163365	51, 52  Moreover, stable complexes between cdk4 and p16Ink4a were detected in several cell types and induction of these binary complexes caused marked inhibition of cdk2 activity by redistribution of cyclin and CKI subunits, particularly those involving p27Kip1 that bind and inhibit cdk2 activity.	bind
28873	1	8437	6	NULL	NULL	0	NULL	cdk4	NULL		forms a complex with	NULL				p16INK4a	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_2_405_s_177	12163365	51, 52  Moreover, stable complexes between cdk4 and p16Ink4a were detected in several cell types and induction of these binary complexes caused marked inhibition of cdk2 activity by redistribution of cyclin and CKI subunits, particularly those involving p27Kip1 that bind and inhibit cdk2 activity.	bind
28875	2	8437	6	NULL	NULL	0	NULL	p27Kip1	NULL		bind	NULL				cdk2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_2_405_s_177	12163365	51, 52  Moreover, stable complexes between cdk4 and p16Ink4a were detected in several cell types and induction of these binary complexes caused marked inhibition of cdk2 activity by redistribution of cyclin and CKI subunits, particularly those involving p27Kip1 that bind and inhibit cdk2 activity.	bind
28876	3	8437	6	NULL	NULL	0	NULL	p27Kip1	NULL		inhibit	NULL				cdk2	NULL	activity of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_2_405_s_177	12163365	51, 52  Moreover, stable complexes between cdk4 and p16Ink4a were detected in several cell types and induction of these binary complexes caused marked inhibition of cdk2 activity by redistribution of cyclin and CKI subunits, particularly those involving p27Kip1 that bind and inhibit cdk2 activity.	bind
28877	4	8437	6	NULL	NULL	0	NULL	statement 1	NULL	induction of	causes	NULL				cdk2 	NULL	inhibiton of;; activity of 			NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_2_405_s_177	12163365	51, 52  Moreover, stable complexes between cdk4 and p16Ink4a were detected in several cell types and induction of these binary complexes caused marked inhibition of cdk2 activity by redistribution of cyclin and CKI subunits, particularly those involving p27Kip1 that bind and inhibit cdk2 activity.	bind
28878	5	8437	6	NULL	NULL	0	NULL	statement 4	NULL		occurs via	NULL				cyclin subunit	NULL	redistribution of 			NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_2_405_s_177	12163365	51, 52  Moreover, stable complexes between cdk4 and p16Ink4a were detected in several cell types and induction of these binary complexes caused marked inhibition of cdk2 activity by redistribution of cyclin and CKI subunits, particularly those involving p27Kip1 that bind and inhibit cdk2 activity.	bind
28879	6	8437	6	NULL	NULL	0	NULL	statement 4	NULL		occurs via	NULL				CKI subunit	NULL	redistribution of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_2_405_s_177	12163365	51, 52  Moreover, stable complexes between cdk4 and p16Ink4a were detected in several cell types and induction of these binary complexes caused marked inhibition of cdk2 activity by redistribution of cyclin and CKI subunits, particularly those involving p27Kip1 that bind and inhibit cdk2 activity.	bind
36122	1	8439	5	13	NULL	NULL	NULL	C/EBP decoy oligonucleotide	NucleicAcid		reduces					intimal hyperplasia	MedicalFinding				NULL	balloon-injured carotid artery of a rabbit atherosclerosis model	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_112	15681294	51,52  The results of a recent study have shown that administration of a C/EBP decoy oligonucleotide into a balloon-injured carotid artery of a rabbit atherosclerosis model reduced intimal hyperplasia and attenuated vascular inflammation accompanied by a complete inhibition of C/EBP protein binding to a consensus C/EBP sequence.	bind
36123	2	8439	5	13	NULL	NULL	NULL	C/EBP decoy oligonucleotide	NucleicAcid		attenuates					vascular inflammation	MedicalFinding				NULL	balloon-injured carotid artery of a rabbit atherosclerosis model	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_112	15681294	51,52  The results of a recent study have shown that administration of a C/EBP decoy oligonucleotide into a balloon-injured carotid artery of a rabbit atherosclerosis model reduced intimal hyperplasia and attenuated vascular inflammation accompanied by a complete inhibition of C/EBP protein binding to a consensus C/EBP sequence.	bind
36124	3	8439	5	13	NULL	NULL	NULL	C/EBP protein	GP		bind							consensus		C/EBP sequence	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_112	15681294	51,52  The results of a recent study have shown that administration of a C/EBP decoy oligonucleotide into a balloon-injured carotid artery of a rabbit atherosclerosis model reduced intimal hyperplasia and attenuated vascular inflammation accompanied by a complete inhibition of C/EBP protein binding to a consensus C/EBP sequence.	bind
36125	4	8439	5	13	NULL	NULL	NULL	statement 1	Process		is followed by					statement 3	Process	inhibition of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_112	15681294	51,52  The results of a recent study have shown that administration of a C/EBP decoy oligonucleotide into a balloon-injured carotid artery of a rabbit atherosclerosis model reduced intimal hyperplasia and attenuated vascular inflammation accompanied by a complete inhibition of C/EBP protein binding to a consensus C/EBP sequence.	bind
36126	5	8439	5	13	NULL	NULL	NULL	statement 2	Process		is followed by					statement 3	Process	inhibition of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_112	15681294	51,52  The results of a recent study have shown that administration of a C/EBP decoy oligonucleotide into a balloon-injured carotid artery of a rabbit atherosclerosis model reduced intimal hyperplasia and attenuated vascular inflammation accompanied by a complete inhibition of C/EBP protein binding to a consensus C/EBP sequence.	bind
28880	1	8439	6	NULL	NULL	0	NULL	C/EBP decoy oligonucleotide	NULL		reduces	NULL				intimal hyperplasia	NULL				NULL	rabbit atherosclerosis model	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_112	15681294	51,52  The results of a recent study have shown that administration of a C/EBP decoy oligonucleotide into a balloon-injured carotid artery of a rabbit atherosclerosis model reduced intimal hyperplasia and attenuated vascular inflammation accompanied by a complete inhibition of C/EBP protein binding to a consensus C/EBP sequence.	bind
28881	2	8439	6	NULL	NULL	0	NULL	C/EBP decoy oligonucleotide	NULL		attenuates	NULL				vascular inflammation	NULL				NULL	rabbit atherosclerosis model	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_112	15681294	51,52  The results of a recent study have shown that administration of a C/EBP decoy oligonucleotide into a balloon-injured carotid artery of a rabbit atherosclerosis model reduced intimal hyperplasia and attenuated vascular inflammation accompanied by a complete inhibition of C/EBP protein binding to a consensus C/EBP sequence.	bind
28882	3	8439	6	NULL	NULL	0	NULL	C/EBP protein	NULL		bind	NULL					NULL	consensus		C/EBP sequence	NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_112	15681294	51,52  The results of a recent study have shown that administration of a C/EBP decoy oligonucleotide into a balloon-injured carotid artery of a rabbit atherosclerosis model reduced intimal hyperplasia and attenuated vascular inflammation accompanied by a complete inhibition of C/EBP protein binding to a consensus C/EBP sequence.	bind
28883	4	8439	6	NULL	NULL	0	NULL	C/EBP decoy oligonucleotide	NULL		inhibits	NULL	completely			statement 3	NULL				NULL	rabbit atherosclerosis model	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_112	15681294	51,52  The results of a recent study have shown that administration of a C/EBP decoy oligonucleotide into a balloon-injured carotid artery of a rabbit atherosclerosis model reduced intimal hyperplasia and attenuated vascular inflammation accompanied by a complete inhibition of C/EBP protein binding to a consensus C/EBP sequence.	bind
36127	1	8440	5	13	NULL	NULL	NULL	EBNA1 protein	GP		bind		constitutively					Epstein-Barr virus		oriP	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_17_3520_s_443	11522821	52       Hsieh,D.-J., Camiolo,S.M. and Yates,J.L. (1993) Constitutive binding of EBNA1 protein to the Epstein-Barr virus replication origin, oriP, with distortion of DNA structure during latent infection.	bind
36128	2	8440	5	13	NULL	NULL	NULL	oriP	NucleicAcid		is					replication origin	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_17_3520_s_443	11522821	52       Hsieh,D.-J., Camiolo,S.M. and Yates,J.L. (1993) Constitutive binding of EBNA1 protein to the Epstein-Barr virus replication origin, oriP, with distortion of DNA structure during latent infection.	bind
36129	3	8440	5	13	NULL	NULL	NULL	statement 1	Process		distorts					DNA	NucleicAcid	structure of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_17_3520_s_443	11522821	52       Hsieh,D.-J., Camiolo,S.M. and Yates,J.L. (1993) Constitutive binding of EBNA1 protein to the Epstein-Barr virus replication origin, oriP, with distortion of DNA structure during latent infection.	bind
28884	1	8440	6	NULL	NULL	0	NULL	EBNA1 protein	NULL		bind	NULL				oriP	NULL	epstein-Barr virus			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_17_3520_s_443	11522821	52       Hsieh,D.-J., Camiolo,S.M. and Yates,J.L. (1993) Constitutive binding of EBNA1 protein to the Epstein-Barr virus replication origin, oriP, with distortion of DNA structure during latent infection.	bind
28885	2	8440	6	NULL	NULL	0	NULL	oriP	NULL		is	NULL				replication origin	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_17_3520_s_443	11522821	52       Hsieh,D.-J., Camiolo,S.M. and Yates,J.L. (1993) Constitutive binding of EBNA1 protein to the Epstein-Barr virus replication origin, oriP, with distortion of DNA structure during latent infection.	bind
36131	1	8441	5	13	NULL	NULL	NULL	estrogen receptor	GP		bind		cooperative					imperfect		estrogen-responsive DNA elements	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_399	11452016	52       Martinez,E., Givel,F. and Wahli,W. (1989) Cooperative binding of estrogen receptor to imperfect estrogen-responsive DNA elements correlates with their synergistic hormone-dependent enhancer activity.	bind
36132	2	8441	5	13	NULL	NULL	NULL	statement 1	Process		coorelates with					estrogen receptor	GP	synergistic;;enhancer activity of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_399	11452016	52       Martinez,E., Givel,F. and Wahli,W. (1989) Cooperative binding of estrogen receptor to imperfect estrogen-responsive DNA elements correlates with their synergistic hormone-dependent enhancer activity.	bind
36133	3	8441	5	13	NULL	NULL	NULL	estrogen receptor	GP	enhancer activity of	dependent on					hormone	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_399	11452016	52       Martinez,E., Givel,F. and Wahli,W. (1989) Cooperative binding of estrogen receptor to imperfect estrogen-responsive DNA elements correlates with their synergistic hormone-dependent enhancer activity.	bind
28886	1	8441	6	NULL	NULL	0	NULL	estrogen receptor	NULL		bind	NULL	cooperatively				NULL	imperfect		estrogen-responsive DNA element	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_399	11452016	52       Martinez,E., Givel,F. and Wahli,W. (1989) Cooperative binding of estrogen receptor to imperfect estrogen-responsive DNA elements correlates with their synergistic hormone-dependent enhancer activity.	bind
28888	2	8441	6	10	NULL	0	NULL	estrogen receptor		enhancer activity of	is dependent on					hormone					NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_399	11452016	52       Martinez,E., Givel,F. and Wahli,W. (1989) Cooperative binding of estrogen receptor to imperfect estrogen-responsive DNA elements correlates with their synergistic hormone-dependent enhancer activity.	bind
28889	3	8441	6	10	NULL	0	NULL	statement 1			correlates with					estrogen receptor		synergistic;;enhancer activity of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_399	11452016	52       Martinez,E., Givel,F. and Wahli,W. (1989) Cooperative binding of estrogen receptor to imperfect estrogen-responsive DNA elements correlates with their synergistic hormone-dependent enhancer activity.	bind
36134	1	8442	5	13	NULL	NULL	NULL	SCF protein	GP		bind					mast cells	Cell	skin			NULL	lesions of patients with urticaria pigmentosa	NULL	NULL	NULL	NULL	gw60_circulation_97_10_971_s_210	9529265	52  Moreover, SCF protein has been detected bound to skin mast cells in lesions of patients with urticaria pigmentosa.	bind
28890	1	8442	6	NULL	NULL	0	NULL	SCF protein	NULL		bind	NULL				mast cells	NULL	skin			NULL	lesions of patients with urticaria pigmentosa	0	NULL	NULL	NULL	gw60_circulation_97_10_971_s_210	9529265	52  Moreover, SCF protein has been detected bound to skin mast cells in lesions of patients with urticaria pigmentosa.	bind
36136	1	8443	5	13	NULL	NULL	NULL	membrane receptor	GP		bind					E2	Chemical				NULL	in endothelial cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_67	12482819	52 Of particular relevance to the vascular system is the observation of a membrane receptor in endothelial cells (ECs) that binds either E2 or E2-BSA rapidly and selectively activates antiapoptotic p38beta MAPK and inhibits proapoptotic p38alpha, leading to upregulation of MAPK-activated protein kinase-2 kinase and phosphorylation of heat shock protein hsp27.	bind
36137	2	8443	5	13	NULL	NULL	NULL	membrane receptor	GP		bind					E2-BSA	Chemical				NULL	in endothelial cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_67	12482819	52 Of particular relevance to the vascular system is the observation of a membrane receptor in endothelial cells (ECs) that binds either E2 or E2-BSA rapidly and selectively activates antiapoptotic p38beta MAPK and inhibits proapoptotic p38alpha, leading to upregulation of MAPK-activated protein kinase-2 kinase and phosphorylation of heat shock protein hsp27.	bind
36138	3	8443	5	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_67	12482819	52 Of particular relevance to the vascular system is the observation of a membrane receptor in endothelial cells (ECs) that binds either E2 or E2-BSA rapidly and selectively activates antiapoptotic p38beta MAPK and inhibits proapoptotic p38alpha, leading to upregulation of MAPK-activated protein kinase-2 kinase and phosphorylation of heat shock protein hsp27.	bind
36139	4	8443	5	13	NULL	NULL	NULL	statement 1	Process		activate		selectively			p38beta MAPK	GP	antiapoptotic			NULL	endothelial cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_67	12482819	52 Of particular relevance to the vascular system is the observation of a membrane receptor in endothelial cells (ECs) that binds either E2 or E2-BSA rapidly and selectively activates antiapoptotic p38beta MAPK and inhibits proapoptotic p38alpha, leading to upregulation of MAPK-activated protein kinase-2 kinase and phosphorylation of heat shock protein hsp27.	bind
36140	5	8443	5	13	NULL	NULL	NULL	statement 1	Process		inhibit		selectively			p38alpha	GP	proapoptotic			NULL	endothelial cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_67	12482819	52 Of particular relevance to the vascular system is the observation of a membrane receptor in endothelial cells (ECs) that binds either E2 or E2-BSA rapidly and selectively activates antiapoptotic p38beta MAPK and inhibits proapoptotic p38alpha, leading to upregulation of MAPK-activated protein kinase-2 kinase and phosphorylation of heat shock protein hsp27.	bind
36141	6	8443	5	13	NULL	NULL	NULL	statement 2	Process		activates		selectively			p38beta MAPK	GP	antiapoptotic			NULL	endothelial cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_67	12482819	52 Of particular relevance to the vascular system is the observation of a membrane receptor in endothelial cells (ECs) that binds either E2 or E2-BSA rapidly and selectively activates antiapoptotic p38beta MAPK and inhibits proapoptotic p38alpha, leading to upregulation of MAPK-activated protein kinase-2 kinase and phosphorylation of heat shock protein hsp27.	bind
36142	7	8443	5	13	NULL	NULL	NULL	statement 2	Process		inhibit		selectively			p38alpha	GP	proapoptotic			NULL	endothelial cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_67	12482819	52 Of particular relevance to the vascular system is the observation of a membrane receptor in endothelial cells (ECs) that binds either E2 or E2-BSA rapidly and selectively activates antiapoptotic p38beta MAPK and inhibits proapoptotic p38alpha, leading to upregulation of MAPK-activated protein kinase-2 kinase and phosphorylation of heat shock protein hsp27.	bind
36143	8	8443	5	13	NULL	NULL	NULL	statement 4	Process		leads to					MAPK-activated protein kinase-2 kinase	GP	upregulation of			NULL	endothelial cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_67	12482819	52 Of particular relevance to the vascular system is the observation of a membrane receptor in endothelial cells (ECs) that binds either E2 or E2-BSA rapidly and selectively activates antiapoptotic p38beta MAPK and inhibits proapoptotic p38alpha, leading to upregulation of MAPK-activated protein kinase-2 kinase and phosphorylation of heat shock protein hsp27.	bind
36144	9	8443	5	13	NULL	NULL	NULL	statement 5	Process		leads to					MAPK-activated protein kinase-2 kinase	GP	upregulation of			NULL	endothelial cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_67	12482819	52 Of particular relevance to the vascular system is the observation of a membrane receptor in endothelial cells (ECs) that binds either E2 or E2-BSA rapidly and selectively activates antiapoptotic p38beta MAPK and inhibits proapoptotic p38alpha, leading to upregulation of MAPK-activated protein kinase-2 kinase and phosphorylation of heat shock protein hsp27.	bind
36145	10	8443	5	13	NULL	NULL	NULL	statement 6	Process		leads to					MAPK-activated protein kinase-2 kinase	GP	upregulation of			NULL	endothelial cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_67	12482819	52 Of particular relevance to the vascular system is the observation of a membrane receptor in endothelial cells (ECs) that binds either E2 or E2-BSA rapidly and selectively activates antiapoptotic p38beta MAPK and inhibits proapoptotic p38alpha, leading to upregulation of MAPK-activated protein kinase-2 kinase and phosphorylation of heat shock protein hsp27.	bind
36146	11	8443	5	13	NULL	NULL	NULL	statement 7	Process		leads to					MAPK-activated protein kinase-2 kinase	GP	upregulation of			NULL	endothelial cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_67	12482819	52 Of particular relevance to the vascular system is the observation of a membrane receptor in endothelial cells (ECs) that binds either E2 or E2-BSA rapidly and selectively activates antiapoptotic p38beta MAPK and inhibits proapoptotic p38alpha, leading to upregulation of MAPK-activated protein kinase-2 kinase and phosphorylation of heat shock protein hsp27.	bind
36147	12	8443	5	13	NULL	NULL	NULL	statement 4	Process		leads to					hsp27	GP	phosphorylation of			NULL	endothelial cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_67	12482819	52 Of particular relevance to the vascular system is the observation of a membrane receptor in endothelial cells (ECs) that binds either E2 or E2-BSA rapidly and selectively activates antiapoptotic p38beta MAPK and inhibits proapoptotic p38alpha, leading to upregulation of MAPK-activated protein kinase-2 kinase and phosphorylation of heat shock protein hsp27.	bind
36148	13	8443	5	13	NULL	NULL	NULL	statement 5	Process		leads to					hsp27	GP	phosphorylation of			NULL	endothelial cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_67	12482819	52 Of particular relevance to the vascular system is the observation of a membrane receptor in endothelial cells (ECs) that binds either E2 or E2-BSA rapidly and selectively activates antiapoptotic p38beta MAPK and inhibits proapoptotic p38alpha, leading to upregulation of MAPK-activated protein kinase-2 kinase and phosphorylation of heat shock protein hsp27.	bind
36149	14	8443	5	13	NULL	NULL	NULL	statement 6	Process		leads to					hsp27	GP	phosphorylation of			NULL	endothelial cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_67	12482819	52 Of particular relevance to the vascular system is the observation of a membrane receptor in endothelial cells (ECs) that binds either E2 or E2-BSA rapidly and selectively activates antiapoptotic p38beta MAPK and inhibits proapoptotic p38alpha, leading to upregulation of MAPK-activated protein kinase-2 kinase and phosphorylation of heat shock protein hsp27.	bind
36150	15	8443	5	13	NULL	NULL	NULL	statement 7	Process		leads to					hsp27	GP	phosphorylation of			NULL	endothelial cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_67	12482819	52 Of particular relevance to the vascular system is the observation of a membrane receptor in endothelial cells (ECs) that binds either E2 or E2-BSA rapidly and selectively activates antiapoptotic p38beta MAPK and inhibits proapoptotic p38alpha, leading to upregulation of MAPK-activated protein kinase-2 kinase and phosphorylation of heat shock protein hsp27.	bind
36151	16	8443	5	13	NULL	NULL	NULL	hsp27	GP		is a type of					heat shock protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_67	12482819	52 Of particular relevance to the vascular system is the observation of a membrane receptor in endothelial cells (ECs) that binds either E2 or E2-BSA rapidly and selectively activates antiapoptotic p38beta MAPK and inhibits proapoptotic p38alpha, leading to upregulation of MAPK-activated protein kinase-2 kinase and phosphorylation of heat shock protein hsp27.	bind
56156	17	8443	5	13	NULL	NULL	NULL	EC	Cell		is					endothelial cell	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_67	12482819	52 Of particular relevance to the vascular system is the observation of a membrane receptor in endothelial cells (ECs) that binds either E2 or E2-BSA rapidly and selectively activates antiapoptotic p38beta MAPK and inhibits proapoptotic p38alpha, leading to upregulation of MAPK-activated protein kinase-2 kinase and phosphorylation of heat shock protein hsp27.	bind
28891	1	8443	6	10	NULL	0	NULL	membrane receptor			bind					E2					NULL	endothelial cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_67	12482819	52 Of particular relevance to the vascular system is the observation of a membrane receptor in endothelial cells (ECs) that binds either E2 or E2-BSA rapidly and selectively activates antiapoptotic p38beta MAPK and inhibits proapoptotic p38alpha, leading to upregulation of MAPK-activated protein kinase-2 kinase and phosphorylation of heat shock protein hsp27.	bind
28892	2	8443	6	10	NULL	0	NULL	membrane receptor			bind					E2-BSA					NULL	endothelial cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_67	12482819	52 Of particular relevance to the vascular system is the observation of a membrane receptor in endothelial cells (ECs) that binds either E2 or E2-BSA rapidly and selectively activates antiapoptotic p38beta MAPK and inhibits proapoptotic p38alpha, leading to upregulation of MAPK-activated protein kinase-2 kinase and phosphorylation of heat shock protein hsp27.	bind
28893	3	8443	6	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_67	12482819	52 Of particular relevance to the vascular system is the observation of a membrane receptor in endothelial cells (ECs) that binds either E2 or E2-BSA rapidly and selectively activates antiapoptotic p38beta MAPK and inhibits proapoptotic p38alpha, leading to upregulation of MAPK-activated protein kinase-2 kinase and phosphorylation of heat shock protein hsp27.	bind
28894	4	8443	6	NULL	NULL	0	NULL	endothelial cell membrane receptor	NULL		activates	NULL	selectively			p38beta MAPK	NULL	antiapoptotic			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_67	12482819	52 Of particular relevance to the vascular system is the observation of a membrane receptor in endothelial cells (ECs) that binds either E2 or E2-BSA rapidly and selectively activates antiapoptotic p38beta MAPK and inhibits proapoptotic p38alpha, leading to upregulation of MAPK-activated protein kinase-2 kinase and phosphorylation of heat shock protein hsp27.	bind
28895	5	8443	6	NULL	NULL	0	NULL	endothelial cell membrane receptor	NULL		inhibits	NULL				p38alpha	NULL	proapoptotic			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_67	12482819	52 Of particular relevance to the vascular system is the observation of a membrane receptor in endothelial cells (ECs) that binds either E2 or E2-BSA rapidly and selectively activates antiapoptotic p38beta MAPK and inhibits proapoptotic p38alpha, leading to upregulation of MAPK-activated protein kinase-2 kinase and phosphorylation of heat shock protein hsp27.	bind
28896	6	8443	6	NULL	NULL	0	NULL	statement 4	NULL		leads to	NULL				MAPK-activated protein kinase-2 kinase	NULL	upregulation of 			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_67	12482819	52 Of particular relevance to the vascular system is the observation of a membrane receptor in endothelial cells (ECs) that binds either E2 or E2-BSA rapidly and selectively activates antiapoptotic p38beta MAPK and inhibits proapoptotic p38alpha, leading to upregulation of MAPK-activated protein kinase-2 kinase and phosphorylation of heat shock protein hsp27.	bind
28897	7	8443	6	NULL	NULL	0	NULL	statement 5	NULL		leads to	NULL				MAPK-activated protein kinase-2 kinase	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_67	12482819	52 Of particular relevance to the vascular system is the observation of a membrane receptor in endothelial cells (ECs) that binds either E2 or E2-BSA rapidly and selectively activates antiapoptotic p38beta MAPK and inhibits proapoptotic p38alpha, leading to upregulation of MAPK-activated protein kinase-2 kinase and phosphorylation of heat shock protein hsp27.	bind
28898	8	8443	6	NULL	NULL	0	NULL	statement 4	NULL		leads to	NULL				hsp27	NULL	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_67	12482819	52 Of particular relevance to the vascular system is the observation of a membrane receptor in endothelial cells (ECs) that binds either E2 or E2-BSA rapidly and selectively activates antiapoptotic p38beta MAPK and inhibits proapoptotic p38alpha, leading to upregulation of MAPK-activated protein kinase-2 kinase and phosphorylation of heat shock protein hsp27.	bind
28899	9	8443	6	NULL	NULL	0	NULL	statement 5	NULL		leads to	NULL				hsp27	NULL	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_67	12482819	52 Of particular relevance to the vascular system is the observation of a membrane receptor in endothelial cells (ECs) that binds either E2 or E2-BSA rapidly and selectively activates antiapoptotic p38beta MAPK and inhibits proapoptotic p38alpha, leading to upregulation of MAPK-activated protein kinase-2 kinase and phosphorylation of heat shock protein hsp27.	bind
28900	10	8443	6	NULL	NULL	0	NULL	hsp27	NULL		is a type of	NULL				heat shock protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_67	12482819	52 Of particular relevance to the vascular system is the observation of a membrane receptor in endothelial cells (ECs) that binds either E2 or E2-BSA rapidly and selectively activates antiapoptotic p38beta MAPK and inhibits proapoptotic p38alpha, leading to upregulation of MAPK-activated protein kinase-2 kinase and phosphorylation of heat shock protein hsp27.	bind
28901	11	8443	6	NULL	NULL	0	NULL	EC	NULL		is	NULL				endothelial cells	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1952_s_67	12482819	52 Of particular relevance to the vascular system is the observation of a membrane receptor in endothelial cells (ECs) that binds either E2 or E2-BSA rapidly and selectively activates antiapoptotic p38beta MAPK and inhibits proapoptotic p38alpha, leading to upregulation of MAPK-activated protein kinase-2 kinase and phosphorylation of heat shock protein hsp27.	bind
36152	1	8444	5	13	NULL	NULL	NULL	apoA-I	GP		bind					ABCA1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_5_720_s_139	12615680	52 These studies imply that binding of apoA-I to ABCA1 may be necessary but not sufficient for stimulating cholesterol efflux.	bind
36153	2	8444	5	13	NULL	NULL	NULL	statement 1	Process		stimulate					cholesterol efflux	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_5_720_s_139	12615680	52 These studies imply that binding of apoA-I to ABCA1 may be necessary but not sufficient for stimulating cholesterol efflux.	bind
36154	3	8444	5	13	NULL	NULL	NULL	statement 1	Process		is necessary for		may be			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_5_720_s_139	12615680	52 These studies imply that binding of apoA-I to ABCA1 may be necessary but not sufficient for stimulating cholesterol efflux.	bind
36155	4	8444	5	13	NULL	NULL	NULL	statement 1	Process		not sufficient for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_5_720_s_139	12615680	52 These studies imply that binding of apoA-I to ABCA1 may be necessary but not sufficient for stimulating cholesterol efflux.	bind
28902	1	8444	6	NULL	NULL	0	NULL	apoA-I	NULL		bind	NULL				ABCA1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_5_720_s_139	12615680	52 These studies imply that binding of apoA-I to ABCA1 may be necessary but not sufficient for stimulating cholesterol efflux.	bind
28903	2	8444	6	NULL	NULL	0	NULL	statement 1	NULL		is necessary for	NULL	may			cholesterol efflux	NULL	stimulation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_5_720_s_139	12615680	52 These studies imply that binding of apoA-I to ABCA1 may be necessary but not sufficient for stimulating cholesterol efflux.	bind
28904	3	8444	6	NULL	NULL	0	NULL	statement 1	NULL		is not sufficient for	NULL				cholesterol efflux	NULL	stimulation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_5_720_s_139	12615680	52 These studies imply that binding of apoA-I to ABCA1 may be necessary but not sufficient for stimulating cholesterol efflux.	bind
36156	1	8445	5	13	NULL	NULL	NULL	lipocalins	GP	tear	bind					lipid ligands	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_7_1514_s_495	11266553	53       Glasgow,B.J., Abduragimov,A.R., Farabakhsh,Z.T., Faull,K.F. and Hubbell,W.L. (1995) Tear lipocalins bind a broad array of lipid ligands.	bind
28905	1	8445	6	10	NULL	0	NULL	lipocalins		tear	bind					lipid ligands					NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_7_1514_s_495	11266553	53       Glasgow,B.J., Abduragimov,A.R., Farabakhsh,Z.T., Faull,K.F. and Hubbell,W.L. (1995) Tear lipocalins bind a broad array of lipid ligands.	bind
36157	1	8446	5	13	NULL	NULL	NULL	53BP1	GP		bind					BRCA1	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_8_6993_s_209	15569676	53BP1 also binds to BRCA1  in vivo; however, it does not bind after ionizing radiation and therefore is unlikely to directly anchor BRCA1 at focal assemblies ( ).	bind
36158	2	8446	5	13	NULL	NULL	NULL	statement 1	Process		does not occur after					ionizing radiation					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_8_6993_s_209	15569676	53BP1 also binds to BRCA1  in vivo; however, it does not bind after ionizing radiation and therefore is unlikely to directly anchor BRCA1 at focal assemblies ( ).	bind
36159	4	8446	5	13	NULL	NULL	NULL	statement 3	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_8_6993_s_209	15569676	53BP1 also binds to BRCA1  in vivo; however, it does not bind after ionizing radiation and therefore is unlikely to directly anchor BRCA1 at focal assemblies ( ).	bind
36160	3	8446	5	13	NULL	NULL	NULL	BRCA1	GP		cannot be anchored at		directly			focal assemblies	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_8_6993_s_209	15569676	53BP1 also binds to BRCA1  in vivo; however, it does not bind after ionizing radiation and therefore is unlikely to directly anchor BRCA1 at focal assemblies ( ).	bind
28906	1	8446	6	NULL	NULL	0	NULL	53BP1	NULL		bind	NULL				BRCA1	NULL				NULL	in vivo	0	NULL	NULL	NULL	gw70_jbiolchem_280_8_6993_s_209	15569676	53BP1 also binds to BRCA1  in vivo; however, it does not bind after ionizing radiation and therefore is unlikely to directly anchor BRCA1 at focal assemblies ( ).	bind
28907	2	8446	6	NULL	NULL	0	NULL	statement 1	NULL		does not occur after	NULL				ionizing radiation	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_8_6993_s_209	15569676	53BP1 also binds to BRCA1  in vivo; however, it does not bind after ionizing radiation and therefore is unlikely to directly anchor BRCA1 at focal assemblies ( ).	bind
28908	3	8446	6	NULL	NULL	0	NULL	BRCA1	NULL		cannot be anchored at	NULL	directly			focal assemblies	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_8_6993_s_209	15569676	53BP1 also binds to BRCA1  in vivo; however, it does not bind after ionizing radiation and therefore is unlikely to directly anchor BRCA1 at focal assemblies ( ).	bind
28909	4	8446	6	NULL	NULL	0	NULL	statement 3	NULL		is due to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_8_6993_s_209	15569676	53BP1 also binds to BRCA1  in vivo; however, it does not bind after ionizing radiation and therefore is unlikely to directly anchor BRCA1 at focal assemblies ( ).	bind
36161	1	8447	5	13	NULL	NULL	NULL	53BP1	GP		bind			BRCT domain		p53	GP		CD		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_9_8051_s_277	15611070	53BP1 binds p53CD via its BRCT domain, which is another general protein recognition motif ( ,  ).	bind
28910	1	8447	6	10	NULL	0	NULL	53BP1	NULL		bind	NULL		BRCT domain		p53	NULL		CD		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_9_8051_s_277	15611070	53BP1 binds p53CD via its BRCT domain, which is another general protein recognition motif ( ,  ).	bind
36162	1	8448	5	13	NULL	NULL	NULL	53BP1	GP		bind			carboxyl terminus		p53	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_24_3387_s_360	9407031	53BP1 binds to a tumor suppressor protein p53 by the two-hybrid method, and the carboxyl terminus of 53BP1 is the site for binding to p53 (Iwabuchi et al. 1994  ).	bind
36163	2	8448	5	13	NULL	NULL	NULL	p53	GP		is a type of					tumor suppressor protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_24_3387_s_360	9407031	53BP1 binds to a tumor suppressor protein p53 by the two-hybrid method, and the carboxyl terminus of 53BP1 is the site for binding to p53 (Iwabuchi et al. 1994  ).	bind
28911	1	8448	6	NULL	NULL	0	NULL	53BP1	NULL		bind	NULL		carboxyl-terminal region		p53	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_11_24_3387_s_360	9407031	53BP1 binds to a tumor suppressor protein p53 by the two-hybrid method, and the carboxyl terminus of 53BP1 is the site for binding to p53 (Iwabuchi et al. 1994  ).	bind
28912	2	8448	6	NULL	NULL	0	NULL	p53	NULL		is a type of	NULL				tumor suppressor protein	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_11_24_3387_s_360	9407031	53BP1 binds to a tumor suppressor protein p53 by the two-hybrid method, and the carboxyl terminus of 53BP1 is the site for binding to p53 (Iwabuchi et al. 1994  ).	bind
36164	1	8449	5	13	NULL	NULL	NULL	53BP1	GP		bind					p53	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_298_5597_1435_s_7	12364621	53BP1 binds to the tumor suppressor protein p53 and has a potential role in DNA damage responses.	bind
36165	2	8449	5	13	NULL	NULL	NULL	p53	GP		is a type of					tumor suppressor protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_298_5597_1435_s_7	12364621	53BP1 binds to the tumor suppressor protein p53 and has a potential role in DNA damage responses.	bind
36166	3	8449	5	13	NULL	NULL	NULL	53BP1	GP		plays a role in		potentially			DNA damage responses	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_298_5597_1435_s_7	12364621	53BP1 binds to the tumor suppressor protein p53 and has a potential role in DNA damage responses.	bind
28913	1	8449	6	NULL	NULL	0	NULL	53BP1	NULL		bind	NULL				p53	NULL				NULL		0	NULL	NULL	NULL	gw60_science_298_5597_1435_s_7	12364621	53BP1 binds to the tumor suppressor protein p53 and has a potential role in DNA damage responses.	bind
28914	2	8449	6	NULL	NULL	0	NULL	p53	NULL		is a type of	NULL				tumor suppressor protein	NULL				NULL		0	NULL	NULL	NULL	gw60_science_298_5597_1435_s_7	12364621	53BP1 binds to the tumor suppressor protein p53 and has a potential role in DNA damage responses.	bind
28915	3	8449	6	NULL	NULL	0	NULL	53BP1	NULL		has a role in	NULL	potential			DNA damage response	NULL				NULL		0	NULL	NULL	NULL	gw60_science_298_5597_1435_s_7	12364621	53BP1 binds to the tumor suppressor protein p53 and has a potential role in DNA damage responses.	bind
36167	1	8450	5	13	NULL	NULL	NULL	53BP1	GP		bind					p53	GP		central DNA-binding domain		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_7_2556_s_2	12640136	53BP1 is a p53 binding protein of unknown function that binds to the central DNA-binding domain of p53.	bind
47883	2	8450	5	13	NULL	NULL	NULL	53BP1 	GP		is a type of					p53 binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_7_2556_s_2	12640136	53BP1 is a p53 binding protein of unknown function that binds to the central DNA-binding domain of p53.	bind
28916	1	8450	6	NULL	NULL	0	NULL	53BP1	NULL		bind	NULL				p53	NULL		central DNA-binding domain		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_7_2556_s_2	12640136	53BP1 is a p53 binding protein of unknown function that binds to the central DNA-binding domain of p53.	bind
47884	2	8450	6	10	NULL	0	NULL	53BP1	NULL		is a type of	NULL				p53 binding protein	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_7_2556_s_2	12640136	53BP1 is a p53 binding protein of unknown function that binds to the central DNA-binding domain of p53.	bind
36168	1	8451	5	13	NULL	NULL	NULL	53BP2	GP		bind					p53C	GP		DNA binding site		NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_2_937_s_87	11782540	53BP2 binds p53C in its DNA binding site, with three loops making the contacts with p53 (ref.  10; Fig.  1).	bind
28917	1	8451	6	NULL	NULL	0	NULL	53BP2	NULL		bind	NULL		three loops		p53C	NULL		DNA binding site		NULL		0	NULL	NULL	NULL	gw60_pnas_99_2_937_s_87	11782540	53BP2 binds p53C in its DNA binding site, with three loops making the contacts with p53 (ref.  10; Fig.  1).	bind
36169	1	8452	5	13	NULL	NULL	NULL	53BP2	GP		bind		tightly			p53C	GP		R273H		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_43_32526_s_112	16887812	53BP2 bound tightly to p53C-R273H, although it is a contact mutant with substantially reduced DNA binding ( ).	bind
47885	2	8452	5	13	NULL	NULL	NULL	 p53C	GP	mutant	bind		reduced	R273H		DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_43_32526_s_112	16887812	53BP2 bound tightly to p53C-R273H, although it is a contact mutant with substantially reduced DNA binding ( ).	bind
28918	1	8452	6	NULL	NULL	0	NULL	53BP2	NULL		bind	NULL	tightly			p53C	NULL	mutant	R273H		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_43_32526_s_112	16887812	53BP2 bound tightly to p53C-R273H, although it is a contact mutant with substantially reduced DNA binding ( ).	bind
28919	2	8452	6	NULL	NULL	0	NULL	p53C	NULL	mutant	has reduced	NULL		R273H		DNA	NULL	binding of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_43_32526_s_112	16887812	53BP2 bound tightly to p53C-R273H, although it is a contact mutant with substantially reduced DNA binding ( ).	bind
36170	1	8453	5	13	NULL	NULL	NULL	estrogen receptor	GP		bind									estrogen-responsive elements	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_405	11452016	54       Ludwig,L.B., Peale,F.V.,Jr, Klinge,C.M., Bambara,R.A., Zain,S. and Hilf,R. (1990) A microtiter well assay for quantitative measurement of estrogen receptor binding to estrogen-responsive elements.	bind
28920	1	8453	6	NULL	NULL	0	NULL	estrogen receptor	NULL		bind	NULL					NULL			estrogen-responsive element	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_405	11452016	54       Ludwig,L.B., Peale,F.V.,Jr, Klinge,C.M., Bambara,R.A., Zain,S. and Hilf,R. (1990) A microtiter well assay for quantitative measurement of estrogen receptor binding to estrogen-responsive elements.	bind
36171	1	8454	5	13	NULL	NULL	NULL	p53	GP		bind					bax	GP			promoter	NULL	myocytes of transgenic mice	NULL	NULL	NULL	NULL	gw60_circulationres_84_7_752_s_311	10205143	54  The quantity of Bax decreased in myocytes of transgenic mice, thus reflecting the attenuation in p53 binding to the bax promoter in these cells.	bind
36172	2	8454	5	13	NULL	NULL	NULL	statement 1	Process	attenuation of	decrease					Bax	GP	quantity of			NULL	myocytes of transgenic mice	NULL	NULL	NULL	NULL	gw60_circulationres_84_7_752_s_311	10205143	54  The quantity of Bax decreased in myocytes of transgenic mice, thus reflecting the attenuation in p53 binding to the bax promoter in these cells.	bind
28921	1	8454	6	NULL	NULL	0	NULL	p53	NULL		bind	NULL				bax	NULL			promoter	NULL	myocytes of transgenic mice	0	NULL	NULL	NULL	gw60_circulationres_84_7_752_s_311	10205143	54  The quantity of Bax decreased in myocytes of transgenic mice, thus reflecting the attenuation in p53 binding to the bax promoter in these cells.	bind
28922	2	8454	6	NULL	NULL	0	NULL	statement 1	NULL	attenuation of	decreases	NULL				Bax	NULL	quantity of			NULL	myocytes of transgenic mice	0	NULL	NULL	NULL	gw60_circulationres_84_7_752_s_311	10205143	54  The quantity of Bax decreased in myocytes of transgenic mice, thus reflecting the attenuation in p53 binding to the bax promoter in these cells.	bind
36733	1	8455	5	13	NULL	NULL	NULL	preheparin LPL	GP		does not bind					endothelium	Cell				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_6_1236_s_117	16574898	54,57  Not bound to the endothelium, it is likely that this preheparin LPL concerns primarily catalytically inactive monomers, probably representing turnover of active dimeric LPL bound to HS-containing proteoglycans as indicated by the group of Olivecrona in 1993.	bind
36735	2	8455	5	13	NULL	NULL	NULL	LPL dimer	GP	active	bind					proteoglycans	GP	HS-containing			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_6_1236_s_117	16574898	54,57  Not bound to the endothelium, it is likely that this preheparin LPL concerns primarily catalytically inactive monomers, probably representing turnover of active dimeric LPL bound to HS-containing proteoglycans as indicated by the group of Olivecrona in 1993.	bind
28923	1	8455	6	10	NULL	0	NULL	LPL dimer		active 	bind					proteoglycans		HS-containing			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_6_1236_s_117	16574898	54,57  Not bound to the endothelium, it is likely that this preheparin LPL concerns primarily catalytically inactive monomers, probably representing turnover of active dimeric LPL bound to HS-containing proteoglycans as indicated by the group of Olivecrona in 1993.	bind
47886	2	8455	6	10	NULL	0	NULL	preheparin LPL	NULL		does not bind	NULL				endothelium	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_6_1236_s_117	16574898	54,57  Not bound to the endothelium, it is likely that this preheparin LPL concerns primarily catalytically inactive monomers, probably representing turnover of active dimeric LPL bound to HS-containing proteoglycans as indicated by the group of Olivecrona in 1993.	bind
36189	1	8456	5	13	NULL	NULL	NULL	54CP	GP		bind					LHCP	GP		third transmembrane domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_17_11622_s_123	9111079	54CP Binds to the Third Transmembrane Domain of LHCP	bind
28924	1	8456	6	NULL	NULL	0	NULL	54CP	NULL		bind	NULL				LHCP	NULL		Third Transmembrane Domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_17_11622_s_123	9111079	54CP Binds to the Third Transmembrane Domain of LHCP	bind
36190	1	8457	5	13	NULL	NULL	NULL	CKIs	GP		inhibit					CDK2	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_369_s_263	11438484	55  ikewise, transforming growth factor-beta growth arrest depends on the inhibition of CDK4 synthesis and further inhibition of CDK2 activity by CKIs. 56 Also, CDK4 disruption was associated with increased binding of p27Kip1 to cyclin E/CDK2 and diminished activation of CDK2 was accompanied by impaired pRb phosphorylation.	bind
36191	2	8457	5	13	NULL	NULL	NULL	CKIs	GP		inhibit					CDK4	GP	synthesis of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_369_s_263	11438484	55  ikewise, transforming growth factor-beta growth arrest depends on the inhibition of CDK4 synthesis and further inhibition of CDK2 activity by CKIs. 56 Also, CDK4 disruption was associated with increased binding of p27Kip1 to cyclin E/CDK2 and diminished activation of CDK2 was accompanied by impaired pRb phosphorylation.	bind
36192	3	8457	5	13	NULL	NULL	NULL	transforming growth factor-beta	GP	growth arrest of	depends on					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_369_s_263	11438484	55  ikewise, transforming growth factor-beta growth arrest depends on the inhibition of CDK4 synthesis and further inhibition of CDK2 activity by CKIs. 56 Also, CDK4 disruption was associated with increased binding of p27Kip1 to cyclin E/CDK2 and diminished activation of CDK2 was accompanied by impaired pRb phosphorylation.	bind
36193	4	8457	5	13	NULL	NULL	NULL	transforming growth factor-beta	GP	growth arrest of	depends on					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_369_s_263	11438484	55  ikewise, transforming growth factor-beta growth arrest depends on the inhibition of CDK4 synthesis and further inhibition of CDK2 activity by CKIs. 56 Also, CDK4 disruption was associated with increased binding of p27Kip1 to cyclin E/CDK2 and diminished activation of CDK2 was accompanied by impaired pRb phosphorylation.	bind
36194	5	8457	5	13	NULL	NULL	NULL	p27Kip1	GP		bind					cyclin E/CDK2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_369_s_263	11438484	55  ikewise, transforming growth factor-beta growth arrest depends on the inhibition of CDK4 synthesis and further inhibition of CDK2 activity by CKIs. 56 Also, CDK4 disruption was associated with increased binding of p27Kip1 to cyclin E/CDK2 and diminished activation of CDK2 was accompanied by impaired pRb phosphorylation.	bind
36195	6	8457	5	13	NULL	NULL	NULL	CDK4	GP	disruption of	is associated with					statement 5	Process	increased			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_369_s_263	11438484	55  ikewise, transforming growth factor-beta growth arrest depends on the inhibition of CDK4 synthesis and further inhibition of CDK2 activity by CKIs. 56 Also, CDK4 disruption was associated with increased binding of p27Kip1 to cyclin E/CDK2 and diminished activation of CDK2 was accompanied by impaired pRb phosphorylation.	bind
36196	7	8457	5	13	NULL	NULL	NULL	CDK2	GP	diminished activation of	is accompanied by					pRb	GP	impaired phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_369_s_263	11438484	55  ikewise, transforming growth factor-beta growth arrest depends on the inhibition of CDK4 synthesis and further inhibition of CDK2 activity by CKIs. 56 Also, CDK4 disruption was associated with increased binding of p27Kip1 to cyclin E/CDK2 and diminished activation of CDK2 was accompanied by impaired pRb phosphorylation.	bind
29030	3	8457	6	10	NULL	0	NULL	transforming growth factor-beta	NULL	growth arrest of	depends on	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_369_s_263	11438484	55  ikewise, transforming growth factor-beta growth arrest depends on the inhibition of CDK4 synthesis and further inhibition of CDK2 activity by CKIs. 56 Also, CDK4 disruption was associated with increased binding of p27Kip1 to cyclin E/CDK2 and diminished activation of CDK2 was accompanied by impaired pRb phosphorylation.	bind
29031	2	8457	6	10	NULL	0	NULL	CKI	NULL		inhibits	NULL				CDK2 	NULL	activity of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_369_s_263	11438484	55  ikewise, transforming growth factor-beta growth arrest depends on the inhibition of CDK4 synthesis and further inhibition of CDK2 activity by CKIs. 56 Also, CDK4 disruption was associated with increased binding of p27Kip1 to cyclin E/CDK2 and diminished activation of CDK2 was accompanied by impaired pRb phosphorylation.	bind
29032	4	8457	6	10	NULL	0	NULL	transforming growth factor-beta	NULL	growth arrest of	depends on	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_369_s_263	11438484	55  ikewise, transforming growth factor-beta growth arrest depends on the inhibition of CDK4 synthesis and further inhibition of CDK2 activity by CKIs. 56 Also, CDK4 disruption was associated with increased binding of p27Kip1 to cyclin E/CDK2 and diminished activation of CDK2 was accompanied by impaired pRb phosphorylation.	bind
29033	5	8457	6	10	NULL	0	NULL	p27Kip1	NULL		bind	NULL				cyclin E/cdk2 complex	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_369_s_263	11438484	55  ikewise, transforming growth factor-beta growth arrest depends on the inhibition of CDK4 synthesis and further inhibition of CDK2 activity by CKIs. 56 Also, CDK4 disruption was associated with increased binding of p27Kip1 to cyclin E/CDK2 and diminished activation of CDK2 was accompanied by impaired pRb phosphorylation.	bind
29034	6	8457	6	10	NULL	0	NULL	CDK4	NULL	disruption of	is associated with	NULL				statement 5	NULL	increased			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_369_s_263	11438484	55  ikewise, transforming growth factor-beta growth arrest depends on the inhibition of CDK4 synthesis and further inhibition of CDK2 activity by CKIs. 56 Also, CDK4 disruption was associated with increased binding of p27Kip1 to cyclin E/CDK2 and diminished activation of CDK2 was accompanied by impaired pRb phosphorylation.	bind
29035	7	8457	6	10	NULL	0	NULL	CDK2	NULL	diminished activation of	is accompanied by	NULL				pRb	NULL	impaired phosphorylation of 			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_1_369_s_263	11438484	55  ikewise, transforming growth factor-beta growth arrest depends on the inhibition of CDK4 synthesis and further inhibition of CDK2 activity by CKIs. 56 Also, CDK4 disruption was associated with increased binding of p27Kip1 to cyclin E/CDK2 and diminished activation of CDK2 was accompanied by impaired pRb phosphorylation.	bind
47887	1	8457	6	10	NULL	0	NULL	CKI	NULL		inhibit	NULL				CDK4	NULL	synthesis of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_1_369_s_263	11438484	55  ikewise, transforming growth factor-beta growth arrest depends on the inhibition of CDK4 synthesis and further inhibition of CDK2 activity by CKIs. 56 Also, CDK4 disruption was associated with increased binding of p27Kip1 to cyclin E/CDK2 and diminished activation of CDK2 was accompanied by impaired pRb phosphorylation.	bind
36182	1	8458	5	13	NULL	NULL	NULL	GDP	Chemical		bind					Rac1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_4_453_s_74	16514078	55 GDP-bound Rac1 or Rac2 does not bind NOXA1, nor does active or inactive Cdc42.	bind
36183	2	8458	5	13	NULL	NULL	NULL	statement 1	GP		does not bind					NOXA1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_4_453_s_74	16514078	55 GDP-bound Rac1 or Rac2 does not bind NOXA1, nor does active or inactive Cdc42.	bind
36184	3	8458	5	13	NULL	NULL	NULL	GDP	Chemical		bind					Rac2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_4_453_s_74	16514078	55 GDP-bound Rac1 or Rac2 does not bind NOXA1, nor does active or inactive Cdc42.	bind
36185	4	8458	5	13	NULL	NULL	NULL	statement 3	GP		does not bind					NOXA1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_4_453_s_74	16514078	55 GDP-bound Rac1 or Rac2 does not bind NOXA1, nor does active or inactive Cdc42.	bind
36186	5	8458	5	13	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_4_453_s_74	16514078	55 GDP-bound Rac1 or Rac2 does not bind NOXA1, nor does active or inactive Cdc42.	bind
36187	6	8458	5	13	NULL	NULL	NULL	Cdc42	GP	active	does not bind					NOXA1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_4_453_s_74	16514078	55 GDP-bound Rac1 or Rac2 does not bind NOXA1, nor does active or inactive Cdc42.	bind
36188	7	8458	5	13	NULL	NULL	NULL	Cdc42	GP	inactive	does not bind					NOXA1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_4_453_s_74	16514078	55 GDP-bound Rac1 or Rac2 does not bind NOXA1, nor does active or inactive Cdc42.	bind
28925	1	8458	6	NULL	NULL	0	NULL	GDP	NULL		bind	NULL				Rac1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_4_453_s_74	16514078	55 GDP-bound Rac1 or Rac2 does not bind NOXA1, nor does active or inactive Cdc42.	bind
28926	2	8458	6	NULL	NULL	0	NULL	GDP	NULL		bind	NULL				Rac2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_4_453_s_74	16514078	55 GDP-bound Rac1 or Rac2 does not bind NOXA1, nor does active or inactive Cdc42.	bind
28927	3	8458	6	NULL	NULL	0	NULL	statement 1	NULL		does not bind	NULL				NOXA1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_4_453_s_74	16514078	55 GDP-bound Rac1 or Rac2 does not bind NOXA1, nor does active or inactive Cdc42.	bind
28928	4	8458	6	NULL	NULL	0	NULL	statement 2	NULL		does not bind	NULL				NOXA1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_4_453_s_74	16514078	55 GDP-bound Rac1 or Rac2 does not bind NOXA1, nor does active or inactive Cdc42.	bind
28929	5	8458	6	NULL	NULL	0	NULL	cdc42	NULL	active	does not bind	NULL				NOXA1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_4_453_s_74	16514078	55 GDP-bound Rac1 or Rac2 does not bind NOXA1, nor does active or inactive Cdc42.	bind
28930	6	8458	6	NULL	NULL	0	NULL	cdc42	NULL	inactive	does not bind	NULL				NOXA1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_4_453_s_74	16514078	55 GDP-bound Rac1 or Rac2 does not bind NOXA1, nor does active or inactive Cdc42.	bind
36303	1	8459	5	13	NULL	NULL	NULL	TNF	GP		bind					TNF-R1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_12_1543_s_116	15217919	55 In this phase, the binding of TNF to TNF-R1 leads to the release of sphingolipid metabolite (stress-induced second messenger) via sphingomyelin degeneration.	bind
36304	2	8459	5	13	NULL	NULL	NULL	statement 1	Process		leads to					sphingolipid metabolite	Chemical	release of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_12_1543_s_116	15217919	55 In this phase, the binding of TNF to TNF-R1 leads to the release of sphingolipid metabolite (stress-induced second messenger) via sphingomyelin degeneration.	bind
36305	5	8459	5	13	NULL	NULL	NULL	sphingolipid metabolite	Chemical		is a type of					statement 3	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_12_1543_s_116	15217919	55 In this phase, the binding of TNF to TNF-R1 leads to the release of sphingolipid metabolite (stress-induced second messenger) via sphingomyelin degeneration.	bind
36306	4	8459	5	13	NULL	NULL	NULL	statement 2	Process		via					sphingomyelin	Chemical	degeneration of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_12_1543_s_116	15217919	55 In this phase, the binding of TNF to TNF-R1 leads to the release of sphingolipid metabolite (stress-induced second messenger) via sphingomyelin degeneration.	bind
47888	3	8459	5	13	NULL	NULL	NULL	stress			induce					secondary messenger	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_12_1543_s_116	15217919	55 In this phase, the binding of TNF to TNF-R1 leads to the release of sphingolipid metabolite (stress-induced second messenger) via sphingomyelin degeneration.	bind
28931	1	8459	6	NULL	NULL	0	NULL	TNF	NULL		bind	NULL				TNF-R1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_12_1543_s_116	15217919	55 In this phase, the binding of TNF to TNF-R1 leads to the release of sphingolipid metabolite (stress-induced second messenger) via sphingomyelin degeneration.	bind
28932	2	8459	6	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				sphingolipid metabolite	NULL	release of			NULL		0	NULL	NULL	NULL	gw70_circulationres_94_12_1543_s_116	15217919	55 In this phase, the binding of TNF to TNF-R1 leads to the release of sphingolipid metabolite (stress-induced second messenger) via sphingomyelin degeneration.	bind
28933	3	8459	6	10	NULL	0	NULL	statement 2	NULL		occurs via	NULL				sphingomyelin 	NULL	degeneration of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_12_1543_s_116	15217919	55 In this phase, the binding of TNF to TNF-R1 leads to the release of sphingolipid metabolite (stress-induced second messenger) via sphingomyelin degeneration.	bind
28934	5	8459	6	10	NULL	0	NULL	sphingolipid metabolite 	NULL		is a type of	NULL				statement 4	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_12_1543_s_116	15217919	55 In this phase, the binding of TNF to TNF-R1 leads to the release of sphingolipid metabolite (stress-induced second messenger) via sphingomyelin degeneration.	bind
47889	4	8459	6	10	NULL	0	NULL	stress	NULL		induce	NULL				secondary messenger	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_12_1543_s_116	15217919	55 In this phase, the binding of TNF to TNF-R1 leads to the release of sphingolipid metabolite (stress-induced second messenger) via sphingomyelin degeneration.	bind
36307	1	8460	5	13	NULL	NULL	NULL	versican	GP		isolated from					ASMCs	Cell	cultured			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_9_1158_s_90	15142969	55 In vitro studies of versican isolated from cultured ASMCs demonstrate that this proteoglycan binds to LDL with saturable kinetics and with a binding affinity for versican of 2.3x10 - 8 mol/L. 56,57  The composition of the CS chains of versican may effect LDL interaction as well.	bind
36308	2	8460	5	13	NULL	NULL	NULL	statement 1	GP		bind					LDL	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_9_1158_s_90	15142969	55 In vitro studies of versican isolated from cultured ASMCs demonstrate that this proteoglycan binds to LDL with saturable kinetics and with a binding affinity for versican of 2.3x10 - 8 mol/L. 56,57  The composition of the CS chains of versican may effect LDL interaction as well.	bind
36309	3	8460	5	13	NULL	NULL	NULL	versican	GP		is a type of					proteoglycan	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_9_1158_s_90	15142969	55 In vitro studies of versican isolated from cultured ASMCs demonstrate that this proteoglycan binds to LDL with saturable kinetics and with a binding affinity for versican of 2.3x10 - 8 mol/L. 56,57  The composition of the CS chains of versican may effect LDL interaction as well.	bind
36310	4	8460	5	13	NULL	NULL	NULL	versican	GP	composition of	effect		may	CS chains		LDL	GP	interaction of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_9_1158_s_90	15142969	55 In vitro studies of versican isolated from cultured ASMCs demonstrate that this proteoglycan binds to LDL with saturable kinetics and with a binding affinity for versican of 2.3x10 - 8 mol/L. 56,57  The composition of the CS chains of versican may effect LDL interaction as well.	bind
29036	1	8460	6	NULL	NULL	0	NULL	versican	NULL		is a type of	NULL				proteoglycan	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_9_1158_s_90	15142969	55 In vitro studies of versican isolated from cultured ASMCs demonstrate that this proteoglycan binds to LDL with saturable kinetics and with a binding affinity for versican of 2.3x10 - 8 mol/L. 56,57  The composition of the CS chains of versican may effect LDL interaction as well.	bind
29037	2	8460	6	NULL	NULL	0	NULL	versican	NULL		bind	NULL				LDL	NULL				NULL	cultured ASMCs	0	NULL	NULL	NULL	gw70_circulationres_94_9_1158_s_90	15142969	55 In vitro studies of versican isolated from cultured ASMCs demonstrate that this proteoglycan binds to LDL with saturable kinetics and with a binding affinity for versican of 2.3x10 - 8 mol/L. 56,57  The composition of the CS chains of versican may effect LDL interaction as well.	bind
36311	1	8461	5	13	NULL	NULL	NULL	Gh	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_5_737_s_144	8620593	56  Interestingly, binding of GTP by Gh inhibits its transglutaminase activity, whereas binding of Ca2+, which is required for transglutaminase activity, prevents GTP binding.	bind
36312	2	8461	5	13	NULL	NULL	NULL	statement 1	Process		inhibit					Gh	GP	transglutaminase activity of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_5_737_s_144	8620593	56  Interestingly, binding of GTP by Gh inhibits its transglutaminase activity, whereas binding of Ca2+, which is required for transglutaminase activity, prevents GTP binding.	bind
36313	3	8461	5	13	NULL	NULL	NULL	Ca2+	Chemical		bind					Gh	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_5_737_s_144	8620593	56  Interestingly, binding of GTP by Gh inhibits its transglutaminase activity, whereas binding of Ca2+, which is required for transglutaminase activity, prevents GTP binding.	bind
36314	4	8461	5	13	NULL	NULL	NULL	statement 3	Process		is required for					Gh	GP	transglutaminase activity of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_5_737_s_144	8620593	56  Interestingly, binding of GTP by Gh inhibits its transglutaminase activity, whereas binding of Ca2+, which is required for transglutaminase activity, prevents GTP binding.	bind
36315	5	8461	5	13	NULL	NULL	NULL	statement 3	Process		prevents					GTP	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_5_737_s_144	8620593	56  Interestingly, binding of GTP by Gh inhibits its transglutaminase activity, whereas binding of Ca2+, which is required for transglutaminase activity, prevents GTP binding.	bind
28935	1	8461	6	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				Gh	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_78_5_737_s_144	8620593	56  Interestingly, binding of GTP by Gh inhibits its transglutaminase activity, whereas binding of Ca2+, which is required for transglutaminase activity, prevents GTP binding.	bind
28937	3	8461	6	10	NULL	0	NULL	statement 1			inhibits					Gh		transglutaminase activity of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_5_737_s_144	8620593	56  Interestingly, binding of GTP by Gh inhibits its transglutaminase activity, whereas binding of Ca2+, which is required for transglutaminase activity, prevents GTP binding.	bind
28938	4	8461	6	NULL	NULL	0	NULL	Ca2+	NULL		bind	NULL				Gh	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_78_5_737_s_144	8620593	56  Interestingly, binding of GTP by Gh inhibits its transglutaminase activity, whereas binding of Ca2+, which is required for transglutaminase activity, prevents GTP binding.	bind
28939	5	8461	6	NULL	NULL	0	NULL	statement 4	NULL		is required for	NULL				transglutaminase activity	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_78_5_737_s_144	8620593	56  Interestingly, binding of GTP by Gh inhibits its transglutaminase activity, whereas binding of Ca2+, which is required for transglutaminase activity, prevents GTP binding.	bind
28940	6	8461	6	NULL	NULL	0	NULL	statement 4	NULL		prevents	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_78_5_737_s_144	8620593	56  Interestingly, binding of GTP by Gh inhibits its transglutaminase activity, whereas binding of Ca2+, which is required for transglutaminase activity, prevents GTP binding.	bind
36316	1	8462	5	13	NULL	NULL	NULL	Egr-1	GP	phosphorylated	bind		less avidly			Sp1	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_3_665_s_146	10079243	56  Phosphorylated Egr-1 binds less avidly to Sp1, resulting in higher levels of free transcription factor and the ability to interact with promoters.	bind
28941	1	8462	6	NULL	NULL	0	NULL	Egr-1	NULL	phosphorylated	bind	NULL	less avidly			Sp1	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_3_665_s_146	10079243	56  Phosphorylated Egr-1 binds less avidly to Sp1, resulting in higher levels of free transcription factor and the ability to interact with promoters.	bind
36320	1	8463	5	13	NULL	NULL	NULL	factor VIIa	GP		bind					tissue factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_265	7586275	56  Therefore, binding of increased factor VIIa and tissue factor could potentially activate the coagulation cascade and generate thrombin continuously, 57  suggesting a significant role of factor VIIa and tissue factor in this animal model.	bind
36321	2	8463	5	13	NULL	NULL	NULL	statement 1	Process	increased	activates		potentially			coagulation cascade	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_265	7586275	56  Therefore, binding of increased factor VIIa and tissue factor could potentially activate the coagulation cascade and generate thrombin continuously, 57  suggesting a significant role of factor VIIa and tissue factor in this animal model.	bind
36322	3	8463	5	13	NULL	NULL	NULL	statement 2	Process		generates		continuously			thrombin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_265	7586275	56  Therefore, binding of increased factor VIIa and tissue factor could potentially activate the coagulation cascade and generate thrombin continuously, 57  suggesting a significant role of factor VIIa and tissue factor in this animal model.	bind
28944	1	8463	6	NULL	NULL	0	NULL	factor VIIa	NULL		bind	NULL				tissue factor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_265	7586275	56  Therefore, binding of increased factor VIIa and tissue factor could potentially activate the coagulation cascade and generate thrombin continuously, 57  suggesting a significant role of factor VIIa and tissue factor in this animal model.	bind
28945	2	8463	6	10	NULL	0	NULL	statement 1		increased	activate		potentially			coagulation cascade					NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_265	7586275	56  Therefore, binding of increased factor VIIa and tissue factor could potentially activate the coagulation cascade and generate thrombin continuously, 57  suggesting a significant role of factor VIIa and tissue factor in this animal model.	bind
28946	3	8463	6	10	NULL	0	NULL	statement 2			generate		continuously			thrombin					NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_10_3041_s_265	7586275	56  Therefore, binding of increased factor VIIa and tissue factor could potentially activate the coagulation cascade and generate thrombin continuously, 57  suggesting a significant role of factor VIIa and tissue factor in this animal model.	bind
36323	1	8464	5	13	NULL	NULL	NULL	LDL	GP	oxidized	activates					MAP kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_141_s_218	9012649	56  These reports suggest that activation of MAP kinase by oxidized LDL may be mediated directly by oxidized LDL binding to a cell-surface receptor that recognizes components of oxidized LDL and then initiates signal transduction.	bind
36324	2	8464	5	13	NULL	NULL	NULL	LDL	GP	oxidized	bind					cell-surface receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_141_s_218	9012649	56  These reports suggest that activation of MAP kinase by oxidized LDL may be mediated directly by oxidized LDL binding to a cell-surface receptor that recognizes components of oxidized LDL and then initiates signal transduction.	bind
36325	3	8464	5	13	NULL	NULL	NULL	statement 2	Process		mediate		directly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_141_s_218	9012649	56  These reports suggest that activation of MAP kinase by oxidized LDL may be mediated directly by oxidized LDL binding to a cell-surface receptor that recognizes components of oxidized LDL and then initiates signal transduction.	bind
36326	4	8464	5	13	NULL	NULL	NULL	cell-surface receptor	GP		recognizes					LDL	GP	components of;;oxidized			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_141_s_218	9012649	56  These reports suggest that activation of MAP kinase by oxidized LDL may be mediated directly by oxidized LDL binding to a cell-surface receptor that recognizes components of oxidized LDL and then initiates signal transduction.	bind
36327	5	8464	5	13	NULL	NULL	NULL	statement 4	Process		initiate					signal transduction	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_141_s_218	9012649	56  These reports suggest that activation of MAP kinase by oxidized LDL may be mediated directly by oxidized LDL binding to a cell-surface receptor that recognizes components of oxidized LDL and then initiates signal transduction.	bind
28947	1	8464	6	NULL	NULL	0	NULL	LDL	NULL	oxidized	activates	NULL				MAP kinase	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_141_s_218	9012649	56  These reports suggest that activation of MAP kinase by oxidized LDL may be mediated directly by oxidized LDL binding to a cell-surface receptor that recognizes components of oxidized LDL and then initiates signal transduction.	bind
28948	2	8464	6	NULL	NULL	0	NULL	LDL	NULL	oxidized	bind	NULL				cell-surface receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_141_s_218	9012649	56  These reports suggest that activation of MAP kinase by oxidized LDL may be mediated directly by oxidized LDL binding to a cell-surface receptor that recognizes components of oxidized LDL and then initiates signal transduction.	bind
28949	3	8464	6	10	NULL	0	NULL	statement 2			mediates		directly			statement 1					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_141_s_218	9012649	56  These reports suggest that activation of MAP kinase by oxidized LDL may be mediated directly by oxidized LDL binding to a cell-surface receptor that recognizes components of oxidized LDL and then initiates signal transduction.	bind
28950	4	8464	6	10	NULL	0	NULL	cell-surface receptors			recognize					LDL		components of;;oxidized			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_141_s_218	9012649	56  These reports suggest that activation of MAP kinase by oxidized LDL may be mediated directly by oxidized LDL binding to a cell-surface receptor that recognizes components of oxidized LDL and then initiates signal transduction.	bind
47891	5	8464	6	10	NULL	0	NULL	statement 4	NULL		initiate	NULL				signal transduction	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_141_s_218	9012649	56  These reports suggest that activation of MAP kinase by oxidized LDL may be mediated directly by oxidized LDL binding to a cell-surface receptor that recognizes components of oxidized LDL and then initiates signal transduction.	bind
36328	1	8465	5	13	NULL	NULL	NULL	SMCs	Cell		uptake					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_1_74_s_232	null	56 57  The conclusion that heparin uptake by SMCs is essential for the inhibitory action of heparin was also reached in a study with heparin-sensitive and heparin-resistant SMCs, in which it was found that upregulation of heparin binding to the SMCs was strongly linked to subsequent internalization and degradation of heparin and was required for the antiproliferative effect of heparin.	bind
36329	2	8465	5	13	NULL	NULL	NULL	statement 1	Process		is essential for					heparin	Chemical	inhibitory action of			NULL	heparin-sensitive SMCs	NULL	NULL	NULL	NULL	gw60_circulationres_84_1_74_s_232	null	56 57  The conclusion that heparin uptake by SMCs is essential for the inhibitory action of heparin was also reached in a study with heparin-sensitive and heparin-resistant SMCs, in which it was found that upregulation of heparin binding to the SMCs was strongly linked to subsequent internalization and degradation of heparin and was required for the antiproliferative effect of heparin.	bind
36722	4	8465	5	13	NULL	NULL	NULL	heparin	Chemical		bind					SMCs	Cell				NULL	heparin-sensitive SMCs	NULL	NULL	NULL	NULL	gw60_circulationres_84_1_74_s_232	null	56 57  The conclusion that heparin uptake by SMCs is essential for the inhibitory action of heparin was also reached in a study with heparin-sensitive and heparin-resistant SMCs, in which it was found that upregulation of heparin binding to the SMCs was strongly linked to subsequent internalization and degradation of heparin and was required for the antiproliferative effect of heparin.	bind
36723	6	8465	5	13	NULL	NULL	NULL	statement 4	Process	upregulation of	is linked to 		strongly			heparin	Chemical	internalization of			NULL	heparin-sensitive SMCs	NULL	NULL	NULL	NULL	gw60_circulationres_84_1_74_s_232	null	56 57  The conclusion that heparin uptake by SMCs is essential for the inhibitory action of heparin was also reached in a study with heparin-sensitive and heparin-resistant SMCs, in which it was found that upregulation of heparin binding to the SMCs was strongly linked to subsequent internalization and degradation of heparin and was required for the antiproliferative effect of heparin.	bind
36724	3	8465	5	13	NULL	NULL	NULL	statement 1	Process		is essential for					heparin	Chemical	inhibitory action of			NULL	heparin-resistant SMCs	NULL	NULL	NULL	NULL	gw60_circulationres_84_1_74_s_232	null	56 57  The conclusion that heparin uptake by SMCs is essential for the inhibitory action of heparin was also reached in a study with heparin-sensitive and heparin-resistant SMCs, in which it was found that upregulation of heparin binding to the SMCs was strongly linked to subsequent internalization and degradation of heparin and was required for the antiproliferative effect of heparin.	bind
36725	5	8465	5	13	NULL	NULL	NULL	heparin	Chemical		bind					SMCs	Cell				NULL	heparin-resistant SMCs	NULL	NULL	NULL	NULL	gw60_circulationres_84_1_74_s_232	null	56 57  The conclusion that heparin uptake by SMCs is essential for the inhibitory action of heparin was also reached in a study with heparin-sensitive and heparin-resistant SMCs, in which it was found that upregulation of heparin binding to the SMCs was strongly linked to subsequent internalization and degradation of heparin and was required for the antiproliferative effect of heparin.	bind
36726	7	8465	5	13	NULL	NULL	NULL	statement 5	Process	upregulation of	is linked to		strongly			heparin	Chemical	internalization of			NULL	heparin-resistant SMCs	NULL	NULL	NULL	NULL	gw60_circulationres_84_1_74_s_232	null	56 57  The conclusion that heparin uptake by SMCs is essential for the inhibitory action of heparin was also reached in a study with heparin-sensitive and heparin-resistant SMCs, in which it was found that upregulation of heparin binding to the SMCs was strongly linked to subsequent internalization and degradation of heparin and was required for the antiproliferative effect of heparin.	bind
36727	8	8465	5	13	NULL	NULL	NULL	statement 4	Process	upregulation of	is linked to		strongly			heparin	Chemical	degradation of			NULL	heparin-sensitive SMCs	NULL	NULL	NULL	NULL	gw60_circulationres_84_1_74_s_232	null	56 57  The conclusion that heparin uptake by SMCs is essential for the inhibitory action of heparin was also reached in a study with heparin-sensitive and heparin-resistant SMCs, in which it was found that upregulation of heparin binding to the SMCs was strongly linked to subsequent internalization and degradation of heparin and was required for the antiproliferative effect of heparin.	bind
36728	9	8465	5	13	NULL	NULL	NULL	statement 5	Process	upregulation of	is linked to		strongly			heparin	Chemical	degradation of			NULL	heparin-resistant SMCs	NULL	NULL	NULL	NULL	gw60_circulationres_84_1_74_s_232	null	56 57  The conclusion that heparin uptake by SMCs is essential for the inhibitory action of heparin was also reached in a study with heparin-sensitive and heparin-resistant SMCs, in which it was found that upregulation of heparin binding to the SMCs was strongly linked to subsequent internalization and degradation of heparin and was required for the antiproliferative effect of heparin.	bind
36729	10	8465	5	13	NULL	NULL	NULL	statement 4	Process	upregulation of	is required for					heparin	Chemical	antiproliferative effect of 			NULL	heparin-sensitive SMCs	NULL	NULL	NULL	NULL	gw60_circulationres_84_1_74_s_232	null	56 57  The conclusion that heparin uptake by SMCs is essential for the inhibitory action of heparin was also reached in a study with heparin-sensitive and heparin-resistant SMCs, in which it was found that upregulation of heparin binding to the SMCs was strongly linked to subsequent internalization and degradation of heparin and was required for the antiproliferative effect of heparin.	bind
36730	11	8465	5	13	NULL	NULL	NULL	statement 4	Process	upregulation of	is required for					heparin	Chemical	antiproliferative effect of			NULL	heparin-resistant SMCs	NULL	NULL	NULL	NULL	gw60_circulationres_84_1_74_s_232	null	56 57  The conclusion that heparin uptake by SMCs is essential for the inhibitory action of heparin was also reached in a study with heparin-sensitive and heparin-resistant SMCs, in which it was found that upregulation of heparin binding to the SMCs was strongly linked to subsequent internalization and degradation of heparin and was required for the antiproliferative effect of heparin.	bind
36731	12	8465	5	13	NULL	NULL	NULL	statement 5	Process	upregulation of	is required for					heparin	Chemical	antiproliferative effect of			NULL	heparin-sensitive SMCs	NULL	NULL	NULL	NULL	gw60_circulationres_84_1_74_s_232	null	56 57  The conclusion that heparin uptake by SMCs is essential for the inhibitory action of heparin was also reached in a study with heparin-sensitive and heparin-resistant SMCs, in which it was found that upregulation of heparin binding to the SMCs was strongly linked to subsequent internalization and degradation of heparin and was required for the antiproliferative effect of heparin.	bind
36732	13	8465	5	13	NULL	NULL	NULL	statement 5	Process	upregulation of	is required for					heparin	Chemical	antiproliferative effect of			NULL	heparin-resistant SMCs	NULL	NULL	NULL	NULL	gw60_circulationres_84_1_74_s_232	null	56 57  The conclusion that heparin uptake by SMCs is essential for the inhibitory action of heparin was also reached in a study with heparin-sensitive and heparin-resistant SMCs, in which it was found that upregulation of heparin binding to the SMCs was strongly linked to subsequent internalization and degradation of heparin and was required for the antiproliferative effect of heparin.	bind
28951	1	8465	6	NULL	NULL	0	NULL	SMC	NULL		plays a role in	NULL				heparin	NULL	uptake of			NULL		0	NULL	NULL	NULL	gw60_circulationres_84_1_74_s_232	null	56 57  The conclusion that heparin uptake by SMCs is essential for the inhibitory action of heparin was also reached in a study with heparin-sensitive and heparin-resistant SMCs, in which it was found that upregulation of heparin binding to the SMCs was strongly linked to subsequent internalization and degradation of heparin and was required for the antiproliferative effect of heparin.	bind
28952	2	8465	6	NULL	NULL	0	NULL	heparin	NULL		exhibits	NULL				inhibitory activity	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_1_74_s_232	null	56 57  The conclusion that heparin uptake by SMCs is essential for the inhibitory action of heparin was also reached in a study with heparin-sensitive and heparin-resistant SMCs, in which it was found that upregulation of heparin binding to the SMCs was strongly linked to subsequent internalization and degradation of heparin and was required for the antiproliferative effect of heparin.	bind
28953	3	8465	6	NULL	NULL	0	NULL	statement 1	NULL		is essential for	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_1_74_s_232	null	56 57  The conclusion that heparin uptake by SMCs is essential for the inhibitory action of heparin was also reached in a study with heparin-sensitive and heparin-resistant SMCs, in which it was found that upregulation of heparin binding to the SMCs was strongly linked to subsequent internalization and degradation of heparin and was required for the antiproliferative effect of heparin.	bind
28954	4	8465	6	NULL	NULL	0	NULL	heparin	NULL		bind	NULL				SMCs	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_1_74_s_232	null	56 57  The conclusion that heparin uptake by SMCs is essential for the inhibitory action of heparin was also reached in a study with heparin-sensitive and heparin-resistant SMCs, in which it was found that upregulation of heparin binding to the SMCs was strongly linked to subsequent internalization and degradation of heparin and was required for the antiproliferative effect of heparin.	bind
28955	5	8465	6	NULL	NULL	0	NULL	statement 4	NULL	upregulation of	is linked to	NULL	strongly			heparin	NULL	internalization of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_1_74_s_232	null	56 57  The conclusion that heparin uptake by SMCs is essential for the inhibitory action of heparin was also reached in a study with heparin-sensitive and heparin-resistant SMCs, in which it was found that upregulation of heparin binding to the SMCs was strongly linked to subsequent internalization and degradation of heparin and was required for the antiproliferative effect of heparin.	bind
28956	6	8465	6	NULL	NULL	0	NULL	statement 4	NULL	upregulation of	is linked to	NULL	strongly			heparin	NULL	degradation of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_1_74_s_232	null	56 57  The conclusion that heparin uptake by SMCs is essential for the inhibitory action of heparin was also reached in a study with heparin-sensitive and heparin-resistant SMCs, in which it was found that upregulation of heparin binding to the SMCs was strongly linked to subsequent internalization and degradation of heparin and was required for the antiproliferative effect of heparin.	bind
28957	7	8465	6	NULL	NULL	0	NULL	heparin	NULL		exhibits	NULL				antiproliferative effect	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_1_74_s_232	null	56 57  The conclusion that heparin uptake by SMCs is essential for the inhibitory action of heparin was also reached in a study with heparin-sensitive and heparin-resistant SMCs, in which it was found that upregulation of heparin binding to the SMCs was strongly linked to subsequent internalization and degradation of heparin and was required for the antiproliferative effect of heparin.	bind
28958	8	8465	6	NULL	NULL	0	NULL	statement 4	NULL	upregulation of	is required for	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_1_74_s_232	null	56 57  The conclusion that heparin uptake by SMCs is essential for the inhibitory action of heparin was also reached in a study with heparin-sensitive and heparin-resistant SMCs, in which it was found that upregulation of heparin binding to the SMCs was strongly linked to subsequent internalization and degradation of heparin and was required for the antiproliferative effect of heparin.	bind
36335	1	8466	5	13	NULL	NULL	NULL	calmodulin	GP		stimulate					type I adenylyl cyclase	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_80_3_297_s_134	9048648	57  Another study showed that the mutation, F503 to R503, in type I adenylyl cyclase within the region corresponding to this peptide abolished calmodulin stimulation of type I adenylyl cyclase, 58  suggesting that this is the calmodulin binding domain of the type I isoform.	bind
36336	2	8466	5	13	NULL	NULL	NULL	type I adenylyl cyclase	GP		is mutated to			F503		type I adenylyl cyclase	GP		R503		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_80_3_297_s_134	9048648	57  Another study showed that the mutation, F503 to R503, in type I adenylyl cyclase within the region corresponding to this peptide abolished calmodulin stimulation of type I adenylyl cyclase, 58  suggesting that this is the calmodulin binding domain of the type I isoform.	bind
36337	3	8466	5	13	NULL	NULL	NULL	statement 2	Process		abolishes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_80_3_297_s_134	9048648	57  Another study showed that the mutation, F503 to R503, in type I adenylyl cyclase within the region corresponding to this peptide abolished calmodulin stimulation of type I adenylyl cyclase, 58  suggesting that this is the calmodulin binding domain of the type I isoform.	bind
36338	4	8466	5	13	NULL	NULL	NULL	type I adenylyl cyclase	GP		is			F503					calmodulin binding domain		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_80_3_297_s_134	9048648	57  Another study showed that the mutation, F503 to R503, in type I adenylyl cyclase within the region corresponding to this peptide abolished calmodulin stimulation of type I adenylyl cyclase, 58  suggesting that this is the calmodulin binding domain of the type I isoform.	bind
29038	1	8466	6	NULL	NULL	0	NULL	type I adenylyl cyclase	NULL		is mutated to	NULL		F503		type I adenylyl cyclase	NULL		R503		NULL		0	NULL	NULL	NULL	gw60_circulationres_80_3_297_s_134	9048648	57  Another study showed that the mutation, F503 to R503, in type I adenylyl cyclase within the region corresponding to this peptide abolished calmodulin stimulation of type I adenylyl cyclase, 58  suggesting that this is the calmodulin binding domain of the type I isoform.	bind
29039	2	8466	6	NULL	NULL	0	NULL	calmodulin	NULL		stimulates	NULL				type I adenylyl cyclase	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_80_3_297_s_134	9048648	57  Another study showed that the mutation, F503 to R503, in type I adenylyl cyclase within the region corresponding to this peptide abolished calmodulin stimulation of type I adenylyl cyclase, 58  suggesting that this is the calmodulin binding domain of the type I isoform.	bind
29040	3	8466	6	NULL	NULL	0	NULL	statement 1	NULL		abolishes	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_80_3_297_s_134	9048648	57  Another study showed that the mutation, F503 to R503, in type I adenylyl cyclase within the region corresponding to this peptide abolished calmodulin stimulation of type I adenylyl cyclase, 58  suggesting that this is the calmodulin binding domain of the type I isoform.	bind
29041	4	8466	6	NULL	NULL	0	NULL	type I adenylyl cyclase	NULL		is	NULL		F503			NULL		calmodulin binding domain		NULL		0	NULL	NULL	NULL	gw60_circulationres_80_3_297_s_134	9048648	57  Another study showed that the mutation, F503 to R503, in type I adenylyl cyclase within the region corresponding to this peptide abolished calmodulin stimulation of type I adenylyl cyclase, 58  suggesting that this is the calmodulin binding domain of the type I isoform.	bind
36339	1	8467	5	13	NULL	NULL	NULL	ARVCF	GP		is					Armadillo-repeat gene deleted in Velo-cardio-facial syndrome	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1431_s_141	16556854	57 In this context, it should be mentioned that also the product of the Armadillo-repeat gene deleted in Velo-cardio-facial syndrome (ARVCF) was demonstrated to be a binding partner of ZO-1 and ZO-2, which in turn differentially regulated ARCF localization to the membrane and the nucleus, respectively.	bind
36340	2	8467	5	13	NULL	NULL	NULL	ARVCF	GP	product of	bind					ZO-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1431_s_141	16556854	57 In this context, it should be mentioned that also the product of the Armadillo-repeat gene deleted in Velo-cardio-facial syndrome (ARVCF) was demonstrated to be a binding partner of ZO-1 and ZO-2, which in turn differentially regulated ARCF localization to the membrane and the nucleus, respectively.	bind
36341	3	8467	5	13	NULL	NULL	NULL	ARVCF	GP	product of	bind					ZO-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1431_s_141	16556854	57 In this context, it should be mentioned that also the product of the Armadillo-repeat gene deleted in Velo-cardio-facial syndrome (ARVCF) was demonstrated to be a binding partner of ZO-1 and ZO-2, which in turn differentially regulated ARCF localization to the membrane and the nucleus, respectively.	bind
36342	4	8467	5	13	NULL	NULL	NULL	ARCF	GP		is localized to					membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1431_s_141	16556854	57 In this context, it should be mentioned that also the product of the Armadillo-repeat gene deleted in Velo-cardio-facial syndrome (ARVCF) was demonstrated to be a binding partner of ZO-1 and ZO-2, which in turn differentially regulated ARCF localization to the membrane and the nucleus, respectively.	bind
36343	5	8467	5	13	NULL	NULL	NULL	ARCF	GP		is localized to					nucleus	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1431_s_141	16556854	57 In this context, it should be mentioned that also the product of the Armadillo-repeat gene deleted in Velo-cardio-facial syndrome (ARVCF) was demonstrated to be a binding partner of ZO-1 and ZO-2, which in turn differentially regulated ARCF localization to the membrane and the nucleus, respectively.	bind
36344	6	8467	5	13	NULL	NULL	NULL	ZO-1	GP		regulates		differentially			statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1431_s_141	16556854	57 In this context, it should be mentioned that also the product of the Armadillo-repeat gene deleted in Velo-cardio-facial syndrome (ARVCF) was demonstrated to be a binding partner of ZO-1 and ZO-2, which in turn differentially regulated ARCF localization to the membrane and the nucleus, respectively.	bind
36345	7	8467	5	13	NULL	NULL	NULL	ZO-2	GP		regulates		differentially			statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1431_s_141	16556854	57 In this context, it should be mentioned that also the product of the Armadillo-repeat gene deleted in Velo-cardio-facial syndrome (ARVCF) was demonstrated to be a binding partner of ZO-1 and ZO-2, which in turn differentially regulated ARCF localization to the membrane and the nucleus, respectively.	bind
28959	1	8467	6	NULL	NULL	0	NULL	Armadillo-repeat gene	NULL		is deleted in	NULL				Velo-cardio-facial syndrome	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1431_s_141	16556854	57 In this context, it should be mentioned that also the product of the Armadillo-repeat gene deleted in Velo-cardio-facial syndrome (ARVCF) was demonstrated to be a binding partner of ZO-1 and ZO-2, which in turn differentially regulated ARCF localization to the membrane and the nucleus, respectively.	bind
28960	2	8467	6	10	NULL	0	NULL	ARVCF	NULL		is	NULL				Armadillo-repeat gene deleted in Velo-cardio-facial syndrome	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1431_s_141	16556854	57 In this context, it should be mentioned that also the product of the Armadillo-repeat gene deleted in Velo-cardio-facial syndrome (ARVCF) was demonstrated to be a binding partner of ZO-1 and ZO-2, which in turn differentially regulated ARCF localization to the membrane and the nucleus, respectively.	bind
28961	3	8467	6	NULL	NULL	0	NULL	Armadillo-repeat gene product	NULL		bind	NULL				ZO-1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1431_s_141	16556854	57 In this context, it should be mentioned that also the product of the Armadillo-repeat gene deleted in Velo-cardio-facial syndrome (ARVCF) was demonstrated to be a binding partner of ZO-1 and ZO-2, which in turn differentially regulated ARCF localization to the membrane and the nucleus, respectively.	bind
28962	4	8467	6	NULL	NULL	0	NULL	Armadillo-repeat gene product	NULL		bind	NULL				ZO-2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1431_s_141	16556854	57 In this context, it should be mentioned that also the product of the Armadillo-repeat gene deleted in Velo-cardio-facial syndrome (ARVCF) was demonstrated to be a binding partner of ZO-1 and ZO-2, which in turn differentially regulated ARCF localization to the membrane and the nucleus, respectively.	bind
28963	5	8467	6	NULL	NULL	0	NULL	ARCF	NULL		localizes to	NULL				membrane	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1431_s_141	16556854	57 In this context, it should be mentioned that also the product of the Armadillo-repeat gene deleted in Velo-cardio-facial syndrome (ARVCF) was demonstrated to be a binding partner of ZO-1 and ZO-2, which in turn differentially regulated ARCF localization to the membrane and the nucleus, respectively.	bind
28964	6	8467	6	NULL	NULL	0	NULL	ARCF	NULL		localizes to	NULL				nucleus	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1431_s_141	16556854	57 In this context, it should be mentioned that also the product of the Armadillo-repeat gene deleted in Velo-cardio-facial syndrome (ARVCF) was demonstrated to be a binding partner of ZO-1 and ZO-2, which in turn differentially regulated ARCF localization to the membrane and the nucleus, respectively.	bind
28965	7	8467	6	10	NULL	0	NULL	statement 3	NULL		regulates	NULL	differentially			statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1431_s_141	16556854	57 In this context, it should be mentioned that also the product of the Armadillo-repeat gene deleted in Velo-cardio-facial syndrome (ARVCF) was demonstrated to be a binding partner of ZO-1 and ZO-2, which in turn differentially regulated ARCF localization to the membrane and the nucleus, respectively.	bind
28966	8	8467	6	10	NULL	0	NULL	statement 3	NULL		regulates	NULL	differentially			statement 6	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1431_s_141	16556854	57 In this context, it should be mentioned that also the product of the Armadillo-repeat gene deleted in Velo-cardio-facial syndrome (ARVCF) was demonstrated to be a binding partner of ZO-1 and ZO-2, which in turn differentially regulated ARCF localization to the membrane and the nucleus, respectively.	bind
28967	9	8467	6	10	NULL	0	NULL	statement 4	NULL		regulates	NULL	differentially			statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1431_s_141	16556854	57 In this context, it should be mentioned that also the product of the Armadillo-repeat gene deleted in Velo-cardio-facial syndrome (ARVCF) was demonstrated to be a binding partner of ZO-1 and ZO-2, which in turn differentially regulated ARCF localization to the membrane and the nucleus, respectively.	bind
28968	10	8467	6	10	NULL	0	NULL	statement 4	NULL		regulates	NULL	differentially			statement 6	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1431_s_141	16556854	57 In this context, it should be mentioned that also the product of the Armadillo-repeat gene deleted in Velo-cardio-facial syndrome (ARVCF) was demonstrated to be a binding partner of ZO-1 and ZO-2, which in turn differentially regulated ARCF localization to the membrane and the nucleus, respectively.	bind
36346	1	8468	5	13	NULL	NULL	NULL	E2F	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2810_s_566	11433027	58       Pagano,M., Durst,M., Joswig,S., Draetta,G. and Jansen-Durr,P. (1992) Binding of the human E2F transcription factor to the retinoblastoma protein but not to cyclin A is abolished in HPV-16-immortalized cells.	bind
36347	2	8468	5	13	NULL	NULL	NULL	E2F	GP	human	bind					retinoblastoma protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2810_s_566	11433027	58       Pagano,M., Durst,M., Joswig,S., Draetta,G. and Jansen-Durr,P. (1992) Binding of the human E2F transcription factor to the retinoblastoma protein but not to cyclin A is abolished in HPV-16-immortalized cells.	bind
36348	3	8468	5	13	NULL	NULL	NULL	E2F	GP	human	does not bind					cyclin A	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2810_s_566	11433027	58       Pagano,M., Durst,M., Joswig,S., Draetta,G. and Jansen-Durr,P. (1992) Binding of the human E2F transcription factor to the retinoblastoma protein but not to cyclin A is abolished in HPV-16-immortalized cells.	bind
36349	4	8468	5	13	NULL	NULL	NULL	statement 2	Process		is abolished in					HPV-16-immortalized cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2810_s_566	11433027	58       Pagano,M., Durst,M., Joswig,S., Draetta,G. and Jansen-Durr,P. (1992) Binding of the human E2F transcription factor to the retinoblastoma protein but not to cyclin A is abolished in HPV-16-immortalized cells.	bind
47892	5	8468	5	13	NULL	NULL	NULL	statement 3	Process		is abolished in					HPV-16-immortalized cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2810_s_566	11433027	58       Pagano,M., Durst,M., Joswig,S., Draetta,G. and Jansen-Durr,P. (1992) Binding of the human E2F transcription factor to the retinoblastoma protein but not to cyclin A is abolished in HPV-16-immortalized cells.	bind
28969	1	8468	6	NULL	NULL	0	NULL	E2F 	NULL	human	bind	NULL				retinoblastoma protein	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2810_s_566	11433027	58       Pagano,M., Durst,M., Joswig,S., Draetta,G. and Jansen-Durr,P. (1992) Binding of the human E2F transcription factor to the retinoblastoma protein but not to cyclin A is abolished in HPV-16-immortalized cells.	bind
28970	2	8468	6	NULL	NULL	0	NULL	E2F	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2810_s_566	11433027	58       Pagano,M., Durst,M., Joswig,S., Draetta,G. and Jansen-Durr,P. (1992) Binding of the human E2F transcription factor to the retinoblastoma protein but not to cyclin A is abolished in HPV-16-immortalized cells.	bind
28971	3	8468	6	NULL	NULL	0	NULL	E2F	NULL	human	does not bind	NULL				cyclin A	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2810_s_566	11433027	58       Pagano,M., Durst,M., Joswig,S., Draetta,G. and Jansen-Durr,P. (1992) Binding of the human E2F transcription factor to the retinoblastoma protein but not to cyclin A is abolished in HPV-16-immortalized cells.	bind
28972	4	8468	6	NULL	NULL	0	NULL	statement 1	NULL		is abolished in	NULL				HPV-16-immortalized cells	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2810_s_566	11433027	58       Pagano,M., Durst,M., Joswig,S., Draetta,G. and Jansen-Durr,P. (1992) Binding of the human E2F transcription factor to the retinoblastoma protein but not to cyclin A is abolished in HPV-16-immortalized cells.	bind
28973	5	8468	6	NULL	NULL	0	NULL	statement 3	NULL		is abolished in	NULL				HPV-16-immortalized cells	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_13_2810_s_566	11433027	58       Pagano,M., Durst,M., Joswig,S., Draetta,G. and Jansen-Durr,P. (1992) Binding of the human E2F transcription factor to the retinoblastoma protein but not to cyclin A is abolished in HPV-16-immortalized cells.	bind
36331	1	8470	5	13	NULL	NULL	NULL	Trx	GP		is					thioredoxin	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1439_s_158	16645155	58,72  In unstressed condition, thioredoxin (Trx) directly binds to ASK1, and inhibits kinase activity.	bind
36332	2	8470	5	13	NULL	NULL	NULL	Trx	GP		bind		directly			ASK1	GP				NULL	unstressed condition	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1439_s_158	16645155	58,72  In unstressed condition, thioredoxin (Trx) directly binds to ASK1, and inhibits kinase activity.	bind
36334	3	8470	5	13	NULL	NULL	NULL	statement 2	Process		inhibit					ASK1	GP	kinase activity of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1439_s_158	16645155	58,72  In unstressed condition, thioredoxin (Trx) directly binds to ASK1, and inhibits kinase activity.	bind
28974	1	8470	6	NULL	NULL	0	NULL	Trx	NULL		bind	NULL	directly			ASK1	NULL				NULL	unstressed condition	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1439_s_158	16645155	58,72  In unstressed condition, thioredoxin (Trx) directly binds to ASK1, and inhibits kinase activity.	bind
28975	2	8470	6	NULL	NULL	0	NULL	Trx	NULL		is	NULL				thioredoxin	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1439_s_158	16645155	58,72  In unstressed condition, thioredoxin (Trx) directly binds to ASK1, and inhibits kinase activity.	bind
28976	3	8470	6	10	NULL	0	NULL	Trx			inhibits					ASK1		kinase activity of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1439_s_158	16645155	58,72  In unstressed condition, thioredoxin (Trx) directly binds to ASK1, and inhibits kinase activity.	bind
36351	2	8471	5	13	NULL	NULL	NULL	decorin	GP		bind		potentially	chondroitin/dermatan sulfate GAG chains		LDL	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_4_519_s_142	9555856	59  Furthermore, decorin and biglycan have chondroitin/dermatan sulfate GAG chains that can potentially bind both LDL and snpPLA2.	bind
36352	1	8471	5	13	NULL	NULL	NULL	decorin	GP		bind		potentially	chondroitin/dermatan sulfate GAG chains		snpPLA2	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_4_519_s_142	9555856	59  Furthermore, decorin and biglycan have chondroitin/dermatan sulfate GAG chains that can potentially bind both LDL and snpPLA2.	bind
36354	4	8471	5	13	NULL	NULL	NULL	biglycan	GP		bind		potentially	chondroitin/dermatan sulfate GAG chains		LDL	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_4_519_s_142	9555856	59  Furthermore, decorin and biglycan have chondroitin/dermatan sulfate GAG chains that can potentially bind both LDL and snpPLA2.	bind
36355	3	8471	5	13	NULL	NULL	NULL	biglycan	GP		bind		potentially	chondroitin/dermatan sulfate GAG chains		snpPLA2	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_4_519_s_142	9555856	59  Furthermore, decorin and biglycan have chondroitin/dermatan sulfate GAG chains that can potentially bind both LDL and snpPLA2.	bind
28977	1	8471	6	NULL	NULL	0	NULL	decorin	NULL		bind	NULL	potentially	chondroitin/dermatan sulfate GAG chains		LDL	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_4_519_s_142	9555856	59  Furthermore, decorin and biglycan have chondroitin/dermatan sulfate GAG chains that can potentially bind both LDL and snpPLA2.	bind
28978	2	8471	6	10	NULL	0	NULL	decorin			bind		potentially	chondroitin/dermatan sulfate GAG chains		snpPLA2					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_4_519_s_142	9555856	59  Furthermore, decorin and biglycan have chondroitin/dermatan sulfate GAG chains that can potentially bind both LDL and snpPLA2.	bind
28979	3	8471	6	10	NULL	0	NULL	biglycan			bind		potentially	chondroitin/dermatan sulfate GAG chains		LDL					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_4_519_s_142	9555856	59  Furthermore, decorin and biglycan have chondroitin/dermatan sulfate GAG chains that can potentially bind both LDL and snpPLA2.	bind
28980	4	8471	6	10	NULL	0	NULL	biglycan			bind		potentially	chondroitin/dermatan sulfate GAG chains		snpPLA2					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_4_519_s_142	9555856	59  Furthermore, decorin and biglycan have chondroitin/dermatan sulfate GAG chains that can potentially bind both LDL and snpPLA2.	bind
36356	1	8472	5	13	NULL	NULL	NULL	helicase	GP		exhibits					ATPase activity	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_35_27145_s_18	10871615	59 protein binds to the helicase, even in the absence of DNA, and stimulates the DNA-dependent and -independent ATPase and DNA unwinding activities of the helicase.	bind
36357	2	8472	5	13	NULL	NULL	NULL	helicase	GP		exhibits					DNA unwinding activity	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_35_27145_s_18	10871615	59 protein binds to the helicase, even in the absence of DNA, and stimulates the DNA-dependent and -independent ATPase and DNA unwinding activities of the helicase.	bind
49157	3	8472	5	13	NULL	NULL	NULL	59 protein	GP		bind					helicase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_35_27145_s_18	10871615	59 protein binds to the helicase, even in the absence of DNA, and stimulates the DNA-dependent and -independent ATPase and DNA unwinding activities of the helicase.	bind
49158	4	8472	5	13	NULL	NULL	NULL	statement 3	Process		in the absence of					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_35_27145_s_18	10871615	59 protein binds to the helicase, even in the absence of DNA, and stimulates the DNA-dependent and -independent ATPase and DNA unwinding activities of the helicase.	bind
49159	5	8472	5	13	NULL	NULL	NULL	59 protein	GP		stimulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_35_27145_s_18	10871615	59 protein binds to the helicase, even in the absence of DNA, and stimulates the DNA-dependent and -independent ATPase and DNA unwinding activities of the helicase.	bind
49160	6	8472	5	13	NULL	NULL	NULL	59 protein	GP		stimulates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_35_27145_s_18	10871615	59 protein binds to the helicase, even in the absence of DNA, and stimulates the DNA-dependent and -independent ATPase and DNA unwinding activities of the helicase.	bind
28981	1	8472	6	NULL	NULL	0	NULL	59 protein	NULL		bind	NULL				helicase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_35_27145_s_18	10871615	59 protein binds to the helicase, even in the absence of DNA, and stimulates the DNA-dependent and -independent ATPase and DNA unwinding activities of the helicase.	bind
28982	2	8472	6	NULL	NULL	0	NULL	statement 1	NULL		occurs in absence of	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_35_27145_s_18	10871615	59 protein binds to the helicase, even in the absence of DNA, and stimulates the DNA-dependent and -independent ATPase and DNA unwinding activities of the helicase.	bind
28983	3	8472	6	NULL	NULL	0	NULL	helicase	NULL		exhibits	NULL				DNA unwinding activity	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_35_27145_s_18	10871615	59 protein binds to the helicase, even in the absence of DNA, and stimulates the DNA-dependent and -independent ATPase and DNA unwinding activities of the helicase.	bind
28984	4	8472	6	NULL	NULL	0	NULL	59 protein	NULL		stimulates	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_35_27145_s_18	10871615	59 protein binds to the helicase, even in the absence of DNA, and stimulates the DNA-dependent and -independent ATPase and DNA unwinding activities of the helicase.	bind
28985	5	8472	6	NULL	NULL	0	NULL	helicase	NULL		exhibits	NULL				ATPase activity	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_35_27145_s_18	10871615	59 protein binds to the helicase, even in the absence of DNA, and stimulates the DNA-dependent and -independent ATPase and DNA unwinding activities of the helicase.	bind
28986	6	8472	6	NULL	NULL	0	NULL	59 protein	NULL		stimulates	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_35_27145_s_18	10871615	59 protein binds to the helicase, even in the absence of DNA, and stimulates the DNA-dependent and -independent ATPase and DNA unwinding activities of the helicase.	bind
36358	1	8473	5	13	NULL	NULL	NULL	Troponin T	GP		bind					tropomyosin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_5_1336_s_103	7648684	59 Troponin T binds to tropomyosin and is responsible for positioning of the troponin complex on the thin filaments.	bind
36359	2	8473	5	13	NULL	NULL	NULL	troponin complex	GP		is positioned on					thin filaments	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_5_1336_s_103	7648684	59 Troponin T binds to tropomyosin and is responsible for positioning of the troponin complex on the thin filaments.	bind
36360	3	8473	5	13	NULL	NULL	NULL	Troponin T	GP		is responsible for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_5_1336_s_103	7648684	59 Troponin T binds to tropomyosin and is responsible for positioning of the troponin complex on the thin filaments.	bind
28987	1	8473	6	NULL	NULL	0	NULL	Troponin T	NULL		bind	NULL				tropomyosin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_5_1336_s_103	7648684	59 Troponin T binds to tropomyosin and is responsible for positioning of the troponin complex on the thin filaments.	bind
29007	2	8473	6	NULL	NULL	0	NULL	troponin complex	NULL		is positioned on	NULL				thin filaments	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_5_1336_s_103	7648684	59 Troponin T binds to tropomyosin and is responsible for positioning of the troponin complex on the thin filaments.	bind
29008	3	8473	6	NULL	NULL	0	NULL	statement 1	NULL		is responsible for	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_5_1336_s_103	7648684	59 Troponin T binds to tropomyosin and is responsible for positioning of the troponin complex on the thin filaments.	bind
36527	1	8474	5	13	NULL	NULL	NULL	RepA	GP		bind					RS sequences	NucleicAcid				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-bacteriol_175_13_8320230_s_17	8320230	5:631-640, 1991), confirm that the binding of RepA  to RS sequences plays a crucial role in the regulation of plasmid replication  and that its binding to IR sequences plays a role in the autoregulation  of RepA expression.	bind
36528	2	8474	5	13	NULL	NULL	NULL	statement 1	Process		plays a role in		crucial			plasmid replication	Process	regulation of			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-bacteriol_175_13_8320230_s_17	8320230	5:631-640, 1991), confirm that the binding of RepA  to RS sequences plays a crucial role in the regulation of plasmid replication  and that its binding to IR sequences plays a role in the autoregulation  of RepA expression.	bind
36529	3	8474	5	13	NULL	NULL	NULL	RepA	GP		bind									IR sequences	NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-bacteriol_175_13_8320230_s_17	8320230	5:631-640, 1991), confirm that the binding of RepA  to RS sequences plays a crucial role in the regulation of plasmid replication  and that its binding to IR sequences plays a role in the autoregulation  of RepA expression.	bind
36530	4	8474	5	13	NULL	NULL	NULL	statement 3	Process		plays a role in		crucial			RepA 	GP	autoregulation of;;expression of			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-bacteriol_175_13_8320230_s_17	8320230	5:631-640, 1991), confirm that the binding of RepA  to RS sequences plays a crucial role in the regulation of plasmid replication  and that its binding to IR sequences plays a role in the autoregulation  of RepA expression.	bind
29134	1	8474	6	NULL	NULL	0	NULL	RepA	NULL		bind	NULL				RS sequences	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-bacteriol_175_13_8320230_s_17	8320230	5:631-640, 1991), confirm that the binding of RepA  to RS sequences plays a crucial role in the regulation of plasmid replication  and that its binding to IR sequences plays a role in the autoregulation  of RepA expression.	bind
29135	2	8474	6	NULL	NULL	0	NULL	statement 1	NULL		plays a role in	NULL				plasmid replication	NULL	regulation of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-bacteriol_175_13_8320230_s_17	8320230	5:631-640, 1991), confirm that the binding of RepA  to RS sequences plays a crucial role in the regulation of plasmid replication  and that its binding to IR sequences plays a role in the autoregulation  of RepA expression.	bind
29139	3	8474	6	NULL	NULL	0	NULL	RepA	NULL		bind	NULL					NULL			IR sequences	NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-bacteriol_175_13_8320230_s_17	8320230	5:631-640, 1991), confirm that the binding of RepA  to RS sequences plays a crucial role in the regulation of plasmid replication  and that its binding to IR sequences plays a role in the autoregulation  of RepA expression.	bind
29140	4	8474	6	NULL	NULL	0	NULL	statement 3	NULL		plays a role in	NULL				RepA	NULL	autoregulation of;; expression of 			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-bacteriol_175_13_8320230_s_17	8320230	5:631-640, 1991), confirm that the binding of RepA  to RS sequences plays a crucial role in the regulation of plasmid replication  and that its binding to IR sequences plays a role in the autoregulation  of RepA expression.	bind
36531	1	8476	5	13	NULL	NULL	NULL	5alpha-DHT	Chemical		is a type of					androgen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_42091_s_15	11514561	5alpha-DHT is a more potent androgen than testosterone in stimulating prostate cancer growth ( 4,  5) and preferentially binds to the androgen receptor (dissociation constant ( K d) for the androgen receptor of 10 11M) ( 6).	bind
36532	2	8476	5	13	NULL	NULL	NULL	testosterone	Chemical		is a type of					androgen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_42091_s_15	11514561	5alpha-DHT is a more potent androgen than testosterone in stimulating prostate cancer growth ( 4,  5) and preferentially binds to the androgen receptor (dissociation constant ( K d) for the androgen receptor of 10 11M) ( 6).	bind
36533	3	8476	5	13	NULL	NULL	NULL	statement 1	Chemical		more potent than					statement 2	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_42091_s_15	11514561	5alpha-DHT is a more potent androgen than testosterone in stimulating prostate cancer growth ( 4,  5) and preferentially binds to the androgen receptor (dissociation constant ( K d) for the androgen receptor of 10 11M) ( 6).	bind
36534	4	8476	5	13	NULL	NULL	NULL	5alpha-DHT	Chemical		stimulate					prostate cancer	MedicalFinding	growth of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_42091_s_15	11514561	5alpha-DHT is a more potent androgen than testosterone in stimulating prostate cancer growth ( 4,  5) and preferentially binds to the androgen receptor (dissociation constant ( K d) for the androgen receptor of 10 11M) ( 6).	bind
36535	5	8476	5	13	NULL	NULL	NULL	testosterone	Chemical		stimulate					prostate cancer	MedicalFinding	growth of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_42091_s_15	11514561	5alpha-DHT is a more potent androgen than testosterone in stimulating prostate cancer growth ( 4,  5) and preferentially binds to the androgen receptor (dissociation constant ( K d) for the androgen receptor of 10 11M) ( 6).	bind
36536	6	8476	5	13	NULL	NULL	NULL	5alpha-DHT	Chemical		bind		preferentially			androgen receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_42091_s_15	11514561	5alpha-DHT is a more potent androgen than testosterone in stimulating prostate cancer growth ( 4,  5) and preferentially binds to the androgen receptor (dissociation constant ( K d) for the androgen receptor of 10 11M) ( 6).	bind
29142	1	8476	6	NULL	NULL	0	NULL	5alpha-DHT	NULL		is a type of	NULL				androgen	NULL	potent			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_45_42091_s_15	11514561	5alpha-DHT is a more potent androgen than testosterone in stimulating prostate cancer growth ( 4,  5) and preferentially binds to the androgen receptor (dissociation constant ( K d) for the androgen receptor of 10 11M) ( 6).	bind
29143	2	8476	6	NULL	NULL	0	NULL	testosterone	NULL		is a type of	NULL				androgen	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_45_42091_s_15	11514561	5alpha-DHT is a more potent androgen than testosterone in stimulating prostate cancer growth ( 4,  5) and preferentially binds to the androgen receptor (dissociation constant ( K d) for the androgen receptor of 10 11M) ( 6).	bind
29144	3	8476	6	NULL	NULL	0	NULL	5alpha-DHT	NULL		stimulates	NULL				prostate cancer	NULL	growth of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_45_42091_s_15	11514561	5alpha-DHT is a more potent androgen than testosterone in stimulating prostate cancer growth ( 4,  5) and preferentially binds to the androgen receptor (dissociation constant ( K d) for the androgen receptor of 10 11M) ( 6).	bind
29145	4	8476	6	NULL	NULL	0	NULL	5alpha-DHT	NULL		bind	NULL	preferentially			androgen receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_45_42091_s_15	11514561	5alpha-DHT is a more potent androgen than testosterone in stimulating prostate cancer growth ( 4,  5) and preferentially binds to the androgen receptor (dissociation constant ( K d) for the androgen receptor of 10 11M) ( 6).	bind
29148	5	8476	6	NULL	NULL	0	NULL	testosterone	NULL		stimulates	NULL				prostate cancer	NULL	growth of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_45_42091_s_15	11514561	5alpha-DHT is a more potent androgen than testosterone in stimulating prostate cancer growth ( 4,  5) and preferentially binds to the androgen receptor (dissociation constant ( K d) for the androgen receptor of 10 11M) ( 6).	bind
29149	6	8476	6	NULL	NULL	0	NULL	statement 3	NULL		is more potent than	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_45_42091_s_15	11514561	5alpha-DHT is a more potent androgen than testosterone in stimulating prostate cancer growth ( 4,  5) and preferentially binds to the androgen receptor (dissociation constant ( K d) for the androgen receptor of 10 11M) ( 6).	bind
36537	1	8477	5	13	NULL	NULL	NULL	 scFv	GP		bind			5B-12B7		NS5B	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_1_593_s_238	11641406	5B-12B7 scFv Binds to NS5B Both in Vitro and in Transfected Cells-- The mAb heavy and light chain variable domains were cloned, and a scFv was assembled to assess the potential of mAb 5B-12B7 to bind to NS5B intracellularly.	bind
36538	2	8477	5	13	NULL	NULL	NULL	 scFv	GP		bind			5B-12B7		NS5B	GP				NULL	transfected cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_1_593_s_238	11641406	5B-12B7 scFv Binds to NS5B Both in Vitro and in Transfected Cells-- The mAb heavy and light chain variable domains were cloned, and a scFv was assembled to assess the potential of mAb 5B-12B7 to bind to NS5B intracellularly.	bind
29152	1	8477	6	NULL	NULL	0	NULL	scFv	NULL		bind	NULL		5B-12B7		NS5B	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_277_1_593_s_238	11641406	5B-12B7 scFv Binds to NS5B Both in Vitro and in Transfected Cells-- The mAb heavy and light chain variable domains were cloned, and a scFv was assembled to assess the potential of mAb 5B-12B7 to bind to NS5B intracellularly.	bind
29154	2	8477	6	NULL	NULL	0	NULL	scFv	NULL		bind	NULL		5B-12B7		NS5B	NULL				NULL	transfected cells	0	NULL	NULL	NULL	gw60_jbiolchem_277_1_593_s_238	11641406	5B-12B7 scFv Binds to NS5B Both in Vitro and in Transfected Cells-- The mAb heavy and light chain variable domains were cloned, and a scFv was assembled to assess the potential of mAb 5B-12B7 to bind to NS5B intracellularly.	bind
36539	1	8478	5	13	NULL	NULL	NULL	5c8 mAb	GP		bind					CD154	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_47_33545_s_78	10559240	5c8 mAb binds to CD154 and blocks the interaction of CD154 with its receptor, CD40 ( 23).	bind
36540	2	8478	5	13	NULL	NULL	NULL	CD154	GP		interact with					CD40	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_47_33545_s_78	10559240	5c8 mAb binds to CD154 and blocks the interaction of CD154 with its receptor, CD40 ( 23).	bind
36541	3	8478	5	13	NULL	NULL	NULL	CD40	GP		is a type of					receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_47_33545_s_78	10559240	5c8 mAb binds to CD154 and blocks the interaction of CD154 with its receptor, CD40 ( 23).	bind
36542	4	8478	5	13	NULL	NULL	NULL	statement 1	Process		block					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_47_33545_s_78	10559240	5c8 mAb binds to CD154 and blocks the interaction of CD154 with its receptor, CD40 ( 23).	bind
29167	1	8478	6	NULL	NULL	0	NULL	5c8 mAb	NULL		bind	NULL				CD154	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_47_33545_s_78	10559240	5c8 mAb binds to CD154 and blocks the interaction of CD154 with its receptor, CD40 ( 23).	bind
29168	2	8478	6	NULL	NULL	0	NULL	CD154	NULL		interacts with	NULL				CD40	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_47_33545_s_78	10559240	5c8 mAb binds to CD154 and blocks the interaction of CD154 with its receptor, CD40 ( 23).	bind
29170	3	8478	6	NULL	NULL	0	NULL	statement 1	NULL		blocks	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_47_33545_s_78	10559240	5c8 mAb binds to CD154 and blocks the interaction of CD154 with its receptor, CD40 ( 23).	bind
36543	1	8479	5	13	NULL	NULL	NULL	5D2 Mabs	GP		bind					LPL	GP				NULL	membrane	NULL	NULL	NULL	NULL	gw70_jlipidres_45_5_859_s_74	14967813	5D2 Mabs bound to LPL on the membrane were then detected using a horseradish peroxidase-linked secondary antibody against mouse and with the ECL-Western blotting analysis system (Amersham).	bind
29171	1	8479	6	NULL	NULL	0	NULL	5D2 Mabs	NULL		bind	NULL				LPL	NULL				NULL	membranes	0	NULL	NULL	NULL	gw70_jlipidres_45_5_859_s_74	14967813	5D2 Mabs bound to LPL on the membrane were then detected using a horseradish peroxidase-linked secondary antibody against mouse and with the ECL-Western blotting analysis system (Amersham).	bind
36544	1	8480	5	13	NULL	NULL	NULL	Shh	GP		bind					Ptc1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_108_4_479_s_62	12860919	5E1 blocks the binding of Shh to Ptc1; it was obtained from Curis Inc and Dr Thomas Jessell (Columbia University) and prepared as purified IgG1 in PBS. 18 Seven days after induction of ischemia, mice were killed.	bind
36545	2	8480	5	13	NULL	NULL	NULL	5E1	GP		block					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_108_4_479_s_62	12860919	5E1 blocks the binding of Shh to Ptc1; it was obtained from Curis Inc and Dr Thomas Jessell (Columbia University) and prepared as purified IgG1 in PBS. 18 Seven days after induction of ischemia, mice were killed.	bind
29172	1	8480	6	NULL	NULL	0	NULL	Shh	NULL		bind	NULL				Ptc1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_108_4_479_s_62	12860919	5E1 blocks the binding of Shh to Ptc1; it was obtained from Curis Inc and Dr Thomas Jessell (Columbia University) and prepared as purified IgG1 in PBS. 18 Seven days after induction of ischemia, mice were killed.	bind
29174	2	8480	6	NULL	NULL	0	NULL	5E1	NULL		blocks	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_108_4_479_s_62	12860919	5E1 blocks the binding of Shh to Ptc1; it was obtained from Curis Inc and Dr Thomas Jessell (Columbia University) and prepared as purified IgG1 in PBS. 18 Seven days after induction of ischemia, mice were killed.	bind
36548	1	8482	5	13	NULL	NULL	NULL	5GG	Chemical		inhibit					AR protein	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_25_7_1109_s_149	14963012	5GG and TF3 inhibit the expression of AR protein   fter T is transformed into DHT by the enzyme 5alpha-reductases, DHT will bind to AR and result in a series of androgen actions.	bind
36549	2	8482	5	13	NULL	NULL	NULL	TF3	Chemical		inhibit					AR protein	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_25_7_1109_s_149	14963012	5GG and TF3 inhibit the expression of AR protein   fter T is transformed into DHT by the enzyme 5alpha-reductases, DHT will bind to AR and result in a series of androgen actions.	bind
36550	3	8482	5	13	NULL	NULL	NULL	T	Chemical		is transformed into					DHT	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_25_7_1109_s_149	14963012	5GG and TF3 inhibit the expression of AR protein   fter T is transformed into DHT by the enzyme 5alpha-reductases, DHT will bind to AR and result in a series of androgen actions.	bind
36551	4	8482	5	13	NULL	NULL	NULL	enzyme 5alpha-reductases	GP		is required for					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_25_7_1109_s_149	14963012	5GG and TF3 inhibit the expression of AR protein   fter T is transformed into DHT by the enzyme 5alpha-reductases, DHT will bind to AR and result in a series of androgen actions.	bind
36552	5	8482	5	13	NULL	NULL	NULL	DHT	Chemical		bind					AR	GP				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_25_7_1109_s_149	14963012	5GG and TF3 inhibit the expression of AR protein   fter T is transformed into DHT by the enzyme 5alpha-reductases, DHT will bind to AR and result in a series of androgen actions.	bind
36553	6	8482	5	13	NULL	NULL	NULL	statement 3	Process		leads to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_25_7_1109_s_149	14963012	5GG and TF3 inhibit the expression of AR protein   fter T is transformed into DHT by the enzyme 5alpha-reductases, DHT will bind to AR and result in a series of androgen actions.	bind
36554	7	8482	5	13	NULL	NULL	NULL	statement 5	Process		results in					androgen actions	Process	series of			NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_25_7_1109_s_149	14963012	5GG and TF3 inhibit the expression of AR protein   fter T is transformed into DHT by the enzyme 5alpha-reductases, DHT will bind to AR and result in a series of androgen actions.	bind
29592	1	8482	6	10	NULL	0	NULL	DHT			bind					AR					NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_25_7_1109_s_149	14963012	5GG and TF3 inhibit the expression of AR protein   fter T is transformed into DHT by the enzyme 5alpha-reductases, DHT will bind to AR and result in a series of androgen actions.	bind
29593	2	8482	6	NULL	NULL	0	NULL	5GG	NULL		inhibit	NULL				AR protein	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_25_7_1109_s_149	14963012	5GG and TF3 inhibit the expression of AR protein   fter T is transformed into DHT by the enzyme 5alpha-reductases, DHT will bind to AR and result in a series of androgen actions.	bind
29594	3	8482	6	NULL	NULL	0	NULL	TF3	NULL		inhibit	NULL				AR protein	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_25_7_1109_s_149	14963012	5GG and TF3 inhibit the expression of AR protein   fter T is transformed into DHT by the enzyme 5alpha-reductases, DHT will bind to AR and result in a series of androgen actions.	bind
29595	4	8482	6	NULL	NULL	0	NULL	statement 1	NULL		results in	NULL				androgen actions	NULL				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_25_7_1109_s_149	14963012	5GG and TF3 inhibit the expression of AR protein   fter T is transformed into DHT by the enzyme 5alpha-reductases, DHT will bind to AR and result in a series of androgen actions.	bind
29596	5	8482	6	NULL	NULL	0	NULL	T	NULL		is transformed into	NULL				DHT	NULL				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_25_7_1109_s_149	14963012	5GG and TF3 inhibit the expression of AR protein   fter T is transformed into DHT by the enzyme 5alpha-reductases, DHT will bind to AR and result in a series of androgen actions.	bind
29597	6	8482	6	NULL	NULL	0	NULL	5alpha-reductases	NULL		carries out	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_25_7_1109_s_149	14963012	5GG and TF3 inhibit the expression of AR protein   fter T is transformed into DHT by the enzyme 5alpha-reductases, DHT will bind to AR and result in a series of androgen actions.	bind
36555	1	8483	5	13	NULL	NULL	NULL	5H2	GP		is a type of					mouse monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_4_844_s_94	9710454	5H2 is a mouse monoclonal antibody which binds to the  COOH-terminal 80-kD segment of the human but not mouse laminin  alpha2.	bind
36556	2	8483	5	13	NULL	NULL	NULL	5H2	GP		bind					laminin alpha2	GP	human	COOH-terminal		NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_4_844_s_94	9710454	5H2 is a mouse monoclonal antibody which binds to the  COOH-terminal 80-kD segment of the human but not mouse laminin  alpha2.	bind
36557	3	8483	5	13	NULL	NULL	NULL	5H2	GP		does not bind					laminin alpha2	GP	mouse	COOH-terminal		NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_4_844_s_94	9710454	5H2 is a mouse monoclonal antibody which binds to the  COOH-terminal 80-kD segment of the human but not mouse laminin  alpha2.	bind
29176	1	8483	6	10	NULL	0	NULL	5H2			bind					laminin alpha2		human	COOH-terminal		NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_4_844_s_94	9710454	5H2 is a mouse monoclonal antibody which binds to the  COOH-terminal 80-kD segment of the human but not mouse laminin  alpha2.	bind
29177	2	8483	6	10	NULL	0	NULL	5H2			does not bind					laminin alpha2		mouse	COOH-terminal		NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_4_844_s_94	9710454	5H2 is a mouse monoclonal antibody which binds to the  COOH-terminal 80-kD segment of the human but not mouse laminin  alpha2.	bind
56157	3	8483	6	10	NULL	0	NULL	5H2			is a type of					mouse monoclonal antibody					NULL		0	NULL	NULL	NULL	gw60_jclininvest_102_4_844_s_94	9710454	5H2 is a mouse monoclonal antibody which binds to the  COOH-terminal 80-kD segment of the human but not mouse laminin  alpha2.	bind
36558	1	8485	5	13	NULL	NULL	NULL	5HT	Chemical		bind					SERTs	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_19_12_4705_s_298	10366604	5HT can bind to SERTs in the absence of Na+ and Cl  (Humphreys et al., 1994  ), but the amine does not translocate.	bind
36559	2	8485	5	13	NULL	NULL	NULL	statement 1	Process		in the absence of					Na+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_19_12_4705_s_298	10366604	5HT can bind to SERTs in the absence of Na+ and Cl  (Humphreys et al., 1994  ), but the amine does not translocate.	bind
36560	3	8485	5	13	NULL	NULL	NULL	statement 1	Process		in the absence of					Cl	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_19_12_4705_s_298	10366604	5HT can bind to SERTs in the absence of Na+ and Cl  (Humphreys et al., 1994  ), but the amine does not translocate.	bind
29179	1	8485	6	NULL	NULL	0	NULL	5HT	NULL		bind	NULL				SERT	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_12_4705_s_298	10366604	5HT can bind to SERTs in the absence of Na+ and Cl  (Humphreys et al., 1994  ), but the amine does not translocate.	bind
29180	2	8485	6	NULL	NULL	0	NULL	statement 1	NULL		occurs in absence of	NULL				Na+	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_12_4705_s_298	10366604	5HT can bind to SERTs in the absence of Na+ and Cl  (Humphreys et al., 1994  ), but the amine does not translocate.	bind
29181	3	8485	6	NULL	NULL	0	NULL	statement 1	NULL		occurs in absence of	NULL				Cl	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_12_4705_s_298	10366604	5HT can bind to SERTs in the absence of Na+ and Cl  (Humphreys et al., 1994  ), but the amine does not translocate.	bind
36561	1	8486	5	13	NULL	NULL	NULL	TFIIIA	GP		bind					5S rDNA	NucleicAcid	naked			NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_21_12169_s_135	9770458	5S DNA ternary complexes could be detected at TFIIIA concentrations only slightly higher than needed for TFIIIA to bind to naked 5S rDNA, and occurred before TFIIIA had bound to all available naked 5S rDNA binding sites (Fig.  4 A).	bind
36562	2	8486	5	13	NULL	NULL	NULL	TFIIIA	GP		bind					5S DNA ternary complexes	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_21_12169_s_135	9770458	5S DNA ternary complexes could be detected at TFIIIA concentrations only slightly higher than needed for TFIIIA to bind to naked 5S rDNA, and occurred before TFIIIA had bound to all available naked 5S rDNA binding sites (Fig.  4 A).	bind
36563	3	8486	5	13	NULL	NULL	NULL	statement 2	Process		occurs before					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_21_12169_s_135	9770458	5S DNA ternary complexes could be detected at TFIIIA concentrations only slightly higher than needed for TFIIIA to bind to naked 5S rDNA, and occurred before TFIIIA had bound to all available naked 5S rDNA binding sites (Fig.  4 A).	bind
29274	1	8486	6	NULL	NULL	0	NULL	TFIIIA	NULL		bind	NULL				5S rDNA	NULL	naked			NULL		0	NULL	NULL	NULL	gw60_pnas_95_21_12169_s_135	9770458	5S DNA ternary complexes could be detected at TFIIIA concentrations only slightly higher than needed for TFIIIA to bind to naked 5S rDNA, and occurred before TFIIIA had bound to all available naked 5S rDNA binding sites (Fig.  4 A).	bind
47894	2	8486	6	10	NULL	0	NULL	TFIIIA	NULL		bind	NULL				5S DNA ternary complexes 	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_21_12169_s_135	9770458	5S DNA ternary complexes could be detected at TFIIIA concentrations only slightly higher than needed for TFIIIA to bind to naked 5S rDNA, and occurred before TFIIIA had bound to all available naked 5S rDNA binding sites (Fig.  4 A).	bind
56158	3	8486	6	10	NULL	0	NULL	statement 2			occurs before					statement 1					NULL		0	NULL	NULL	NULL	gw60_pnas_95_21_12169_s_135	9770458	5S DNA ternary complexes could be detected at TFIIIA concentrations only slightly higher than needed for TFIIIA to bind to naked 5S rDNA, and occurred before TFIIIA had bound to all available naked 5S rDNA binding sites (Fig.  4 A).	bind
36564	1	8487	5	13	NULL	NULL	NULL	5S	GP		is a type of					mouse monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0580-0599_biotechnol-appl-biochem_43_pt-2_16253117_s_4	16253117	5S is  a mouse monoclonal antibody that binds to HBsAg with very high affinity.	bind
36565	2	8487	5	13	NULL	NULL	NULL	5S	GP		bind		high affinity			HBsAg	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0580-0599_biotechnol-appl-biochem_43_pt-2_16253117_s_4	16253117	5S is  a mouse monoclonal antibody that binds to HBsAg with very high affinity.	bind
29275	1	8487	6	10	NULL	0	NULL	5S 			bind		high affinity			HbsAg					NULL		NULL	NULL	NULL	NULL	abs-batch0580-0599_biotechnol-appl-biochem_43_pt-2_16253117_s_4	16253117	5S is  a mouse monoclonal antibody that binds to HBsAg with very high affinity.	bind
47895	2	8487	6	10	NULL	0	NULL	5S	NULL		is a type of	NULL				 mouse monoclonal antibody	NULL				NULL		0	NULL	NULL	NULL	abs-batch0580-0599_biotechnol-appl-biochem_43_pt-2_16253117_s_4	16253117	5S is  a mouse monoclonal antibody that binds to HBsAg with very high affinity.	bind
36566	1	8488	5	13	NULL	NULL	NULL	5S rDNA	NucleicAcid		complex with					histone octamers	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_21_12169_s_153	9770458	5S rDNA ternary complexes, no TFIIIA binding to 5S rDNA complexed with histone octamers could be detected (Fig.  4 B).	bind
36567	2	8488	5	13	NULL	NULL	NULL	TFIIIA	GP		does not bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_21_12169_s_153	9770458	5S rDNA ternary complexes, no TFIIIA binding to 5S rDNA complexed with histone octamers could be detected (Fig.  4 B).	bind
29277	1	8488	6	NULL	NULL	0	NULL	5S rDNA	NULL		complexes with	NULL				histone octamers	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_21_12169_s_153	9770458	5S rDNA ternary complexes, no TFIIIA binding to 5S rDNA complexed with histone octamers could be detected (Fig.  4 B).	bind
29278	2	8488	6	NULL	NULL	0	NULL	TFIIIA	NULL		does not bind	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_21_12169_s_153	9770458	5S rDNA ternary complexes, no TFIIIA binding to 5S rDNA complexed with histone octamers could be detected (Fig.  4 B).	bind
36711	1	8490	5	13	NULL	NULL	NULL	5S rRNA	NucleicAcid		bind					viral protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_1_166_s_37	10592212	5S rRNA binds the viral protein ( 32) and enhances the methionyl- and isoleucyl-tRNA synthetase activities by direct interactions with MetRS and tRNAMet in the macromolecular aminoacyl-tRNA synthetase complex ( 33).	bind
36712	2	8490	5	13	NULL	NULL	NULL	statement 1	GP		interact with		directly			MetRS	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_1_166_s_37	10592212	5S rRNA binds the viral protein ( 32) and enhances the methionyl- and isoleucyl-tRNA synthetase activities by direct interactions with MetRS and tRNAMet in the macromolecular aminoacyl-tRNA synthetase complex ( 33).	bind
36713	3	8490	5	13	NULL	NULL	NULL	statement 1	GP		interact with		directly			tRNAMet	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_1_166_s_37	10592212	5S rRNA binds the viral protein ( 32) and enhances the methionyl- and isoleucyl-tRNA synthetase activities by direct interactions with MetRS and tRNAMet in the macromolecular aminoacyl-tRNA synthetase complex ( 33).	bind
36714	4	8490	5	13	NULL	NULL	NULL	statement 2	Process		occurs in					aminoacyl-tRNA synthetase complex	GP	macromolecular			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_1_166_s_37	10592212	5S rRNA binds the viral protein ( 32) and enhances the methionyl- and isoleucyl-tRNA synthetase activities by direct interactions with MetRS and tRNAMet in the macromolecular aminoacyl-tRNA synthetase complex ( 33).	bind
36715	5	8490	5	13	NULL	NULL	NULL	statement 3	Process		occurs in					aminoacyl-tRNA synthetase complex	GP	macromolecular			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_1_166_s_37	10592212	5S rRNA binds the viral protein ( 32) and enhances the methionyl- and isoleucyl-tRNA synthetase activities by direct interactions with MetRS and tRNAMet in the macromolecular aminoacyl-tRNA synthetase complex ( 33).	bind
36716	6	8490	5	13	NULL	NULL	NULL	statement 1	Process		enhance					methionyl-tRNA synthetase	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_1_166_s_37	10592212	5S rRNA binds the viral protein ( 32) and enhances the methionyl- and isoleucyl-tRNA synthetase activities by direct interactions with MetRS and tRNAMet in the macromolecular aminoacyl-tRNA synthetase complex ( 33).	bind
36717	7	8490	5	13	NULL	NULL	NULL	statement 1	Process		enhance					isoleucyl-tRNA synthetase	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_1_166_s_37	10592212	5S rRNA binds the viral protein ( 32) and enhances the methionyl- and isoleucyl-tRNA synthetase activities by direct interactions with MetRS and tRNAMet in the macromolecular aminoacyl-tRNA synthetase complex ( 33).	bind
36718	8	8490	5	13	NULL	NULL	NULL	statement 2	Process		leads to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_1_166_s_37	10592212	5S rRNA binds the viral protein ( 32) and enhances the methionyl- and isoleucyl-tRNA synthetase activities by direct interactions with MetRS and tRNAMet in the macromolecular aminoacyl-tRNA synthetase complex ( 33).	bind
36719	9	8490	5	13	NULL	NULL	NULL	statement 2	Process		leads to					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_1_166_s_37	10592212	5S rRNA binds the viral protein ( 32) and enhances the methionyl- and isoleucyl-tRNA synthetase activities by direct interactions with MetRS and tRNAMet in the macromolecular aminoacyl-tRNA synthetase complex ( 33).	bind
36720	10	8490	5	13	NULL	NULL	NULL	statement 3	Process		leads to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_1_166_s_37	10592212	5S rRNA binds the viral protein ( 32) and enhances the methionyl- and isoleucyl-tRNA synthetase activities by direct interactions with MetRS and tRNAMet in the macromolecular aminoacyl-tRNA synthetase complex ( 33).	bind
36721	11	8490	5	13	NULL	NULL	NULL	statement 3	Process		leads to					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_1_166_s_37	10592212	5S rRNA binds the viral protein ( 32) and enhances the methionyl- and isoleucyl-tRNA synthetase activities by direct interactions with MetRS and tRNAMet in the macromolecular aminoacyl-tRNA synthetase complex ( 33).	bind
29281	1	8490	6	NULL	NULL	0	NULL	5S rRNA	NULL		bind	NULL				viral protein	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_1_166_s_37	10592212	5S rRNA binds the viral protein ( 32) and enhances the methionyl- and isoleucyl-tRNA synthetase activities by direct interactions with MetRS and tRNAMet in the macromolecular aminoacyl-tRNA synthetase complex ( 33).	bind
29282	2	8490	6	NULL	NULL	0	NULL	5S rRNA	NULL		interacts with	NULL	directly			MetRS	NULL				NULL	macromolecular aminoacyl-tRNA synthetase complex	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_1_166_s_37	10592212	5S rRNA binds the viral protein ( 32) and enhances the methionyl- and isoleucyl-tRNA synthetase activities by direct interactions with MetRS and tRNAMet in the macromolecular aminoacyl-tRNA synthetase complex ( 33).	bind
29283	3	8490	6	NULL	NULL	0	NULL	5S rRNA	NULL		interacts with	NULL	directly			tRNAMet	NULL				NULL	macromolecular aminoacyl-tRNA synthetase complex	0	NULL	NULL	NULL	gw60_nucleicacidsres_28_1_166_s_37	10592212	5S rRNA binds the viral protein ( 32) and enhances the methionyl- and isoleucyl-tRNA synthetase activities by direct interactions with MetRS and tRNAMet in the macromolecular aminoacyl-tRNA synthetase complex ( 33).	bind
29286	4	8490	6	NULL	NULL	0	NULL	statement 2	NULL		enhances	NULL				methionyl tRNA synthetase	NULL	activity of			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_1_166_s_37	10592212	5S rRNA binds the viral protein ( 32) and enhances the methionyl- and isoleucyl-tRNA synthetase activities by direct interactions with MetRS and tRNAMet in the macromolecular aminoacyl-tRNA synthetase complex ( 33).	bind
29288	5	8490	6	NULL	NULL	0	NULL	statement 3	NULL		enhances	NULL				isoleucyl-tRNA synthetase	NULL	activity of			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_1_166_s_37	10592212	5S rRNA binds the viral protein ( 32) and enhances the methionyl- and isoleucyl-tRNA synthetase activities by direct interactions with MetRS and tRNAMet in the macromolecular aminoacyl-tRNA synthetase complex ( 33).	bind
36568	1	8491	5	13	NULL	NULL	NULL	tmRNA	NucleicAcid		bind					alanyl-tRNA synthetase	GP	Escherichia coli			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_7_1602_s_156	11266563	6       Barends,S., Wower,J. and Kraal,B. (2000) Kinetic parameters for tmRNA binding to alanyl-tRNA synthetase and elongation factor Tu from  Escherichia coli.	bind
36569	2	8491	5	13	NULL	NULL	NULL	tmRNA	NucleicAcid		bind					Tu	GP	Escherichia coli			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_7_1602_s_156	11266563	6       Barends,S., Wower,J. and Kraal,B. (2000) Kinetic parameters for tmRNA binding to alanyl-tRNA synthetase and elongation factor Tu from  Escherichia coli.	bind
47896	3	8491	5	13	NULL	NULL	NULL	Tu	GP		is a type of					elongation factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_7_1602_s_156	11266563	6       Barends,S., Wower,J. and Kraal,B. (2000) Kinetic parameters for tmRNA binding to alanyl-tRNA synthetase and elongation factor Tu from  Escherichia coli.	bind
29289	1	8491	6	10	NULL	0	NULL	tmRNA			bind					alanyl-tRNA synthetase		Escherichia coli			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_7_1602_s_156	11266563	6       Barends,S., Wower,J. and Kraal,B. (2000) Kinetic parameters for tmRNA binding to alanyl-tRNA synthetase and elongation factor Tu from  Escherichia coli.	bind
29290	2	8491	6	10	NULL	0	NULL	tmRNA			bind					Tu		Escherichia coli			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_7_1602_s_156	11266563	6       Barends,S., Wower,J. and Kraal,B. (2000) Kinetic parameters for tmRNA binding to alanyl-tRNA synthetase and elongation factor Tu from  Escherichia coli.	bind
29291	3	8491	6	NULL	NULL	0	NULL	Tu	NULL		is a type of	NULL				elongation factor	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_7_1602_s_156	11266563	6       Barends,S., Wower,J. and Kraal,B. (2000) Kinetic parameters for tmRNA binding to alanyl-tRNA synthetase and elongation factor Tu from  Escherichia coli.	bind
36570	1	8494	5	13	NULL	NULL	NULL	fibrin(ogen)	GP		bind					ECs	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1544_s_180	8977460	6  32 42 43 45 46 47 48  The lack of association between FBG and ECs contradicts these other studies, in which specific binding of FBG to ECs was demonstrated; however, the lack of FBG binding to ECs in our study most likely reflects differences in the methods used to study the heparin-dependent binding of fibrin(ogen) to ECs.	bind
36571	2	8494	5	13	NULL	NULL	NULL	statement 1	Process		is dependent on					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1544_s_180	8977460	6  32 42 43 45 46 47 48  The lack of association between FBG and ECs contradicts these other studies, in which specific binding of FBG to ECs was demonstrated; however, the lack of FBG binding to ECs in our study most likely reflects differences in the methods used to study the heparin-dependent binding of fibrin(ogen) to ECs.	bind
29292	1	8494	6	NULL	NULL	0	NULL	fibrinogen	NULL		bind	NULL				EC	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1544_s_180	8977460	6  32 42 43 45 46 47 48  The lack of association between FBG and ECs contradicts these other studies, in which specific binding of FBG to ECs was demonstrated; however, the lack of FBG binding to ECs in our study most likely reflects differences in the methods used to study the heparin-dependent binding of fibrin(ogen) to ECs.	bind
29293	2	8494	6	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				heparin	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1544_s_180	8977460	6  32 42 43 45 46 47 48  The lack of association between FBG and ECs contradicts these other studies, in which specific binding of FBG to ECs was demonstrated; however, the lack of FBG binding to ECs in our study most likely reflects differences in the methods used to study the heparin-dependent binding of fibrin(ogen) to ECs.	bind
36572	1	8495	5	13	NULL	NULL	NULL	zymogen factor X	GP		bind					Mac-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_27	10510057	6  7  Binding of the zymogen factor X to Mac-1 results in the acceleration of its conversion to activated factor Xa and thus constitutes an alternative pathway for the initiation of the coagulation serine protease cascade.	bind
36573	2	8495	5	13	NULL	NULL	NULL	zymogen factor X	GP		is converted to					factor Xa	GP	activated			NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_27	10510057	6  7  Binding of the zymogen factor X to Mac-1 results in the acceleration of its conversion to activated factor Xa and thus constitutes an alternative pathway for the initiation of the coagulation serine protease cascade.	bind
36574	3	8495	5	13	NULL	NULL	NULL	statement 1	Process		accelerate					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_27	10510057	6  7  Binding of the zymogen factor X to Mac-1 results in the acceleration of its conversion to activated factor Xa and thus constitutes an alternative pathway for the initiation of the coagulation serine protease cascade.	bind
36575	4	8495	5	13	NULL	NULL	NULL	statement 3	Process		initiates					coagulation serine protease cascade	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_27	10510057	6  7  Binding of the zymogen factor X to Mac-1 results in the acceleration of its conversion to activated factor Xa and thus constitutes an alternative pathway for the initiation of the coagulation serine protease cascade.	bind
29294	1	8495	6	NULL	NULL	0	NULL	zymogen factor X	NULL		bind	NULL				Mac-1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_27	10510057	6  7  Binding of the zymogen factor X to Mac-1 results in the acceleration of its conversion to activated factor Xa and thus constitutes an alternative pathway for the initiation of the coagulation serine protease cascade.	bind
29295	2	8495	6	NULL	NULL	0	NULL	zymogen factor X	NULL		is converted to	NULL				factor Xa	NULL	activated			NULL		0	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_27	10510057	6  7  Binding of the zymogen factor X to Mac-1 results in the acceleration of its conversion to activated factor Xa and thus constitutes an alternative pathway for the initiation of the coagulation serine protease cascade.	bind
29296	3	8495	6	NULL	NULL	0	NULL	statement 1	NULL		accelerates 	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_27	10510057	6  7  Binding of the zymogen factor X to Mac-1 results in the acceleration of its conversion to activated factor Xa and thus constitutes an alternative pathway for the initiation of the coagulation serine protease cascade.	bind
29297	4	8495	6	NULL	NULL	0	NULL	statement 3	NULL		initiates	NULL				coagulation serine protease cascade	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_27	10510057	6  7  Binding of the zymogen factor X to Mac-1 results in the acceleration of its conversion to activated factor Xa and thus constitutes an alternative pathway for the initiation of the coagulation serine protease cascade.	bind
36576	1	8496	5	13	NULL	NULL	NULL	p53	GP		bind					bax	GP			promoter	NULL	myocytes	NULL	NULL	NULL	NULL	gw60_circulationres_88_3_298_s_214	11179197	6  7  p53 binding to the bax promoter is enhanced, and the amount of Bax protein in myocytes increases several fold.	bind
36577	2	8496	5	13	NULL	NULL	NULL	statement 1	Process	enhanced	results in					Bax protein	GP	increased			NULL	myocytes	NULL	NULL	NULL	NULL	gw60_circulationres_88_3_298_s_214	11179197	6  7  p53 binding to the bax promoter is enhanced, and the amount of Bax protein in myocytes increases several fold.	bind
29298	1	8496	6	10	NULL	0	NULL	p53			bind					bax				promoter	NULL	myocytes	NULL	NULL	NULL	NULL	gw60_circulationres_88_3_298_s_214	11179197	6  7  p53 binding to the bax promoter is enhanced, and the amount of Bax protein in myocytes increases several fold.	bind
47897	2	8496	6	10	NULL	0	NULL	statement 1	NULL		results in	NULL				Bax protein	NULL	increased			NULL	myocytes	0	NULL	NULL	NULL	gw60_circulationres_88_3_298_s_214	11179197	6  7  p53 binding to the bax promoter is enhanced, and the amount of Bax protein in myocytes increases several fold.	bind
36691	1	8497	5	13	NULL	NULL	NULL	Aogen	GP		is a limiting factor in					Ang II	GP	synthesis of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_3_298_s_35	11179197	6  7 26 27 28  Aogen is the limiting factor in the synthesis of Ang II, 28  and binding to AT1 conditions myocyte growth and death.	bind
36692	2	8497	5	13	NULL	NULL	NULL	Aogen	GP		bind					AT1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_3_298_s_35	11179197	6  7 26 27 28  Aogen is the limiting factor in the synthesis of Ang II, 28  and binding to AT1 conditions myocyte growth and death.	bind
36693	3	8497	5	13	NULL	NULL	NULL	statement 2	Process		conditions					myocyte	Cell	growth of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_3_298_s_35	11179197	6  7 26 27 28  Aogen is the limiting factor in the synthesis of Ang II, 28  and binding to AT1 conditions myocyte growth and death.	bind
36694	4	8497	5	13	NULL	NULL	NULL	statement 2	Process		conditions					myocyte	Cell	death of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_3_298_s_35	11179197	6  7 26 27 28  Aogen is the limiting factor in the synthesis of Ang II, 28  and binding to AT1 conditions myocyte growth and death.	bind
29299	1	8497	6	NULL	NULL	0	NULL	Aogen	NULL		is the limiting factor for	NULL				Ang II	NULL	synthesis of			NULL		0	NULL	NULL	NULL	gw60_circulationres_88_3_298_s_35	11179197	6  7 26 27 28  Aogen is the limiting factor in the synthesis of Ang II, 28  and binding to AT1 conditions myocyte growth and death.	bind
29300	2	8497	6	NULL	NULL	0	NULL	Aogen	NULL		bind	NULL				AT1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_88_3_298_s_35	11179197	6  7 26 27 28  Aogen is the limiting factor in the synthesis of Ang II, 28  and binding to AT1 conditions myocyte growth and death.	bind
29301	3	8497	6	NULL	NULL	0	NULL	statement 2	NULL		conditions	NULL				myocyte	NULL	growth of 			NULL		0	NULL	NULL	NULL	gw60_circulationres_88_3_298_s_35	11179197	6  7 26 27 28  Aogen is the limiting factor in the synthesis of Ang II, 28  and binding to AT1 conditions myocyte growth and death.	bind
29302	4	8497	6	NULL	NULL	0	NULL	statement 2	NULL		conditions	NULL				myocyte	NULL	death of 			NULL		0	NULL	NULL	NULL	gw60_circulationres_88_3_298_s_35	11179197	6  7 26 27 28  Aogen is the limiting factor in the synthesis of Ang II, 28  and binding to AT1 conditions myocyte growth and death.	bind
36695	1	8498	5	13	NULL	NULL	NULL	THM	GP		bind					thrombin	GP				NULL	normal arteries	NULL	NULL	NULL	NULL	gw60_circulation_102_3_332_s_110	10899098	6  7 8  In normal arteries, THM binds thrombin and prevents PAR activation while also catalytically activating protein C, which adds additional antithrombotic and anti-inflammatory effects.	bind
36696	2	8498	5	13	NULL	NULL	NULL	statement 1	Process		prevents					PAR	GP	activation of			NULL	normal arteries	NULL	NULL	NULL	NULL	gw60_circulation_102_3_332_s_110	10899098	6  7 8  In normal arteries, THM binds thrombin and prevents PAR activation while also catalytically activating protein C, which adds additional antithrombotic and anti-inflammatory effects.	bind
36697	3	8498	5	13	NULL	NULL	NULL	statement 1	Process		activates		catalytically			protein C	GP				NULL	normal arteries	NULL	NULL	NULL	NULL	gw60_circulation_102_3_332_s_110	10899098	6  7 8  In normal arteries, THM binds thrombin and prevents PAR activation while also catalytically activating protein C, which adds additional antithrombotic and anti-inflammatory effects.	bind
36698	4	8498	5	13	NULL	NULL	NULL	statement 3	Process		results in					antithrombotic effect	Process				NULL	normal arteries	NULL	NULL	NULL	NULL	gw60_circulation_102_3_332_s_110	10899098	6  7 8  In normal arteries, THM binds thrombin and prevents PAR activation while also catalytically activating protein C, which adds additional antithrombotic and anti-inflammatory effects.	bind
36699	5	8498	5	13	NULL	NULL	NULL	statement 3	Process		results in					anti-inflammatory effect	Process				NULL	normal arteries	NULL	NULL	NULL	NULL	gw60_circulation_102_3_332_s_110	10899098	6  7 8  In normal arteries, THM binds thrombin and prevents PAR activation while also catalytically activating protein C, which adds additional antithrombotic and anti-inflammatory effects.	bind
29303	1	8498	6	10	NULL	0	NULL	THM	NULL		bind	NULL				thrombin	NULL				NULL	 normal arteries	NULL	NULL	NULL	NULL	gw60_circulation_102_3_332_s_110	10899098	6  7 8  In normal arteries, THM binds thrombin and prevents PAR activation while also catalytically activating protein C, which adds additional antithrombotic and anti-inflammatory effects.	bind
29304	2	8498	6	10	NULL	0	NULL	statement 1	NULL		prevents	NULL				PAR	NULL	activation of			NULL	 normal arteries	NULL	NULL	NULL	NULL	gw60_circulation_102_3_332_s_110	10899098	6  7 8  In normal arteries, THM binds thrombin and prevents PAR activation while also catalytically activating protein C, which adds additional antithrombotic and anti-inflammatory effects.	bind
29305	3	8498	6	10	NULL	0	NULL	THM	NULL		activates	NULL	catalytically			protein C	NULL				NULL	 normal arteries	NULL	NULL	NULL	NULL	gw60_circulation_102_3_332_s_110	10899098	6  7 8  In normal arteries, THM binds thrombin and prevents PAR activation while also catalytically activating protein C, which adds additional antithrombotic and anti-inflammatory effects.	bind
29306	4	8498	6	10	NULL	0	NULL	statement 3	NULL		provides	NULL				antithrombotic effect	NULL				NULL	 normal arteries	NULL	NULL	NULL	NULL	gw60_circulation_102_3_332_s_110	10899098	6  7 8  In normal arteries, THM binds thrombin and prevents PAR activation while also catalytically activating protein C, which adds additional antithrombotic and anti-inflammatory effects.	bind
29307	5	8498	6	10	NULL	0	NULL	statement 3	NULL		provides	NULL				anti-inflammatory effects	NULL				NULL	 normal arteries	NULL	NULL	NULL	NULL	gw60_circulation_102_3_332_s_110	10899098	6  7 8  In normal arteries, THM binds thrombin and prevents PAR activation while also catalytically activating protein C, which adds additional antithrombotic and anti-inflammatory effects.	bind
36700	1	8499	5	13	NULL	NULL	NULL	apoB-100	GP	single copies of	bind					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_1013_s_30	9633945	6  Even though single copies of apoB-100 and apoE bind to the LDL receptor with similar affinities, lipoproteins with multiple copies of apoE bind to multiple LDL receptors, increasing the affinity of the lipoprotein-receptor interaction.	bind
36701	2	8499	5	13	NULL	NULL	NULL	apoE	GP	single copies of	bind					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_1013_s_30	9633945	6  Even though single copies of apoB-100 and apoE bind to the LDL receptor with similar affinities, lipoproteins with multiple copies of apoE bind to multiple LDL receptors, increasing the affinity of the lipoprotein-receptor interaction.	bind
36702	3	8499	5	13	NULL	NULL	NULL	statement 1	Process		similar affinity to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_1013_s_30	9633945	6  Even though single copies of apoB-100 and apoE bind to the LDL receptor with similar affinities, lipoproteins with multiple copies of apoE bind to multiple LDL receptors, increasing the affinity of the lipoprotein-receptor interaction.	bind
36703	4	8499	5	13	NULL	NULL	NULL	lipoproteins	GP		contains					apoE	GP	multiple copies of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_1013_s_30	9633945	6  Even though single copies of apoB-100 and apoE bind to the LDL receptor with similar affinities, lipoproteins with multiple copies of apoE bind to multiple LDL receptors, increasing the affinity of the lipoprotein-receptor interaction.	bind
36704	5	8499	5	13	NULL	NULL	NULL	statement 4	GP		bind					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_1013_s_30	9633945	6  Even though single copies of apoB-100 and apoE bind to the LDL receptor with similar affinities, lipoproteins with multiple copies of apoE bind to multiple LDL receptors, increasing the affinity of the lipoprotein-receptor interaction.	bind
36705	6	8499	5	13	NULL	NULL	NULL	statement 5	Process		increase					lipoprotein-receptor 	GP	affinity of;;interaction of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_1013_s_30	9633945	6  Even though single copies of apoB-100 and apoE bind to the LDL receptor with similar affinities, lipoproteins with multiple copies of apoE bind to multiple LDL receptors, increasing the affinity of the lipoprotein-receptor interaction.	bind
29308	1	8499	6	NULL	NULL	0	NULL	apoB-100	NULL		bind	NULL				LDL receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_1013_s_30	9633945	6  Even though single copies of apoB-100 and apoE bind to the LDL receptor with similar affinities, lipoproteins with multiple copies of apoE bind to multiple LDL receptors, increasing the affinity of the lipoprotein-receptor interaction.	bind
29309	2	8499	6	NULL	NULL	0	NULL	apoE	NULL		bind	NULL				LDL receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_1013_s_30	9633945	6  Even though single copies of apoB-100 and apoE bind to the LDL receptor with similar affinities, lipoproteins with multiple copies of apoE bind to multiple LDL receptors, increasing the affinity of the lipoprotein-receptor interaction.	bind
47898	3	8499	6	10	NULL	0	NULL	statement 1	NULL	affinity of	similar to	NULL				statement 2	NULL	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_1013_s_30	9633945	6  Even though single copies of apoB-100 and apoE bind to the LDL receptor with similar affinities, lipoproteins with multiple copies of apoE bind to multiple LDL receptors, increasing the affinity of the lipoprotein-receptor interaction.	bind
47899	4	8499	6	10	NULL	0	NULL	lipoproteins	NULL		contains	NULL				apoE	NULL	multiple copies of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_1013_s_30	9633945	6  Even though single copies of apoB-100 and apoE bind to the LDL receptor with similar affinities, lipoproteins with multiple copies of apoE bind to multiple LDL receptors, increasing the affinity of the lipoprotein-receptor interaction.	bind
47900	5	8499	6	10	NULL	0	NULL	statement 4	NULL		bind	NULL				LDL receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_1013_s_30	9633945	6  Even though single copies of apoB-100 and apoE bind to the LDL receptor with similar affinities, lipoproteins with multiple copies of apoE bind to multiple LDL receptors, increasing the affinity of the lipoprotein-receptor interaction.	bind
47901	6	8499	6	10	NULL	0	NULL	statement 5	NULL		increase	NULL				 lipoprotein-receptor	NULL	affinity of;;interaction of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_6_1013_s_30	9633945	6  Even though single copies of apoB-100 and apoE bind to the LDL receptor with similar affinities, lipoproteins with multiple copies of apoE bind to multiple LDL receptors, increasing the affinity of the lipoprotein-receptor interaction.	bind
36706	1	8500	5	13	NULL	NULL	NULL	heparin	Chemical	soluble	bind					Mac-1	GP				NULL	patients treated with heparin	NULL	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_168	10510057	6  Furthermore, binding of soluble heparin to Mac-1 in patients treated with heparin may inhibit leukocyte adhesion, which was recently described to be partially mediated by binding of Mac-1 to heparin-like structures bound on endothelial cells.	bind
36707	2	8500	5	13	NULL	NULL	NULL	statement 1	Process		inhibit		may			leukocyte 	Cell	adhesion of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_168	10510057	6  Furthermore, binding of soluble heparin to Mac-1 in patients treated with heparin may inhibit leukocyte adhesion, which was recently described to be partially mediated by binding of Mac-1 to heparin-like structures bound on endothelial cells.	bind
36708	3	8500	5	13	NULL	NULL	NULL	heparin-like structures	Chemical		bind					endothelial cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_168	10510057	6  Furthermore, binding of soluble heparin to Mac-1 in patients treated with heparin may inhibit leukocyte adhesion, which was recently described to be partially mediated by binding of Mac-1 to heparin-like structures bound on endothelial cells.	bind
36709	4	8500	5	13	NULL	NULL	NULL	Mac-1	GP		bind					statement 3	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_168	10510057	6  Furthermore, binding of soluble heparin to Mac-1 in patients treated with heparin may inhibit leukocyte adhesion, which was recently described to be partially mediated by binding of Mac-1 to heparin-like structures bound on endothelial cells.	bind
36710	5	8500	5	13	NULL	NULL	NULL	statement 2	Process		mediated by		partially			statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_168	10510057	6  Furthermore, binding of soluble heparin to Mac-1 in patients treated with heparin may inhibit leukocyte adhesion, which was recently described to be partially mediated by binding of Mac-1 to heparin-like structures bound on endothelial cells.	bind
29310	1	8500	6	NULL	NULL	0	NULL	heparin	NULL	soluble	bind	NULL				Mac-1	NULL				NULL	patients treated with heparin	0	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_168	10510057	6  Furthermore, binding of soluble heparin to Mac-1 in patients treated with heparin may inhibit leukocyte adhesion, which was recently described to be partially mediated by binding of Mac-1 to heparin-like structures bound on endothelial cells.	bind
29311	2	8500	6	NULL	NULL	0	NULL	statement 1	NULL		inhibits	NULL	may			leukocyte	NULL	adhesion of 			NULL		0	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_168	10510057	6  Furthermore, binding of soluble heparin to Mac-1 in patients treated with heparin may inhibit leukocyte adhesion, which was recently described to be partially mediated by binding of Mac-1 to heparin-like structures bound on endothelial cells.	bind
29312	3	8500	6	NULL	NULL	0	NULL	heparin-like structures	NULL		bind	NULL				endothelial cells	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_168	10510057	6  Furthermore, binding of soluble heparin to Mac-1 in patients treated with heparin may inhibit leukocyte adhesion, which was recently described to be partially mediated by binding of Mac-1 to heparin-like structures bound on endothelial cells.	bind
29313	4	8500	6	NULL	NULL	0	NULL	Mac-1	NULL		bind	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_168	10510057	6  Furthermore, binding of soluble heparin to Mac-1 in patients treated with heparin may inhibit leukocyte adhesion, which was recently described to be partially mediated by binding of Mac-1 to heparin-like structures bound on endothelial cells.	bind
29314	5	8500	6	NULL	NULL	0	NULL	statement 2	NULL		is mediated by	NULL	partially			statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_168	10510057	6  Furthermore, binding of soluble heparin to Mac-1 in patients treated with heparin may inhibit leukocyte adhesion, which was recently described to be partially mediated by binding of Mac-1 to heparin-like structures bound on endothelial cells.	bind
33563	1	8501	5	13	NULL	NULL	NULL	KY3	Chemical		bind					VDR	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_23_2867_s_24	11104746	6  KY3 has  20 times higher affinity for VDR than 1,25(OH)2D3 and does not bind to the transport protein vitamin D - binding protein.	bind
33564	2	8501	5	13	NULL	NULL	NULL	KY3	Chemical		bind					1,25(OH)2D3	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_23_2867_s_24	11104746	6  KY3 has  20 times higher affinity for VDR than 1,25(OH)2D3 and does not bind to the transport protein vitamin D - binding protein.	bind
33565	3	8501	5	13	NULL	NULL	NULL	statement 1	Chemical		high affinity than					statement 2	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_23_2867_s_24	11104746	6  KY3 has  20 times higher affinity for VDR than 1,25(OH)2D3 and does not bind to the transport protein vitamin D - binding protein.	bind
33566	4	8501	5	13	NULL	NULL	NULL	KY3	Chemical		does not bind					vitamin D - binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_23_2867_s_24	11104746	6  KY3 has  20 times higher affinity for VDR than 1,25(OH)2D3 and does not bind to the transport protein vitamin D - binding protein.	bind
55723	5	8501	5	13	NULL	NULL	NULL	vitamin D - binding protein	GP		is a type of 					transport protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_23_2867_s_24	11104746	6  KY3 has  20 times higher affinity for VDR than 1,25(OH)2D3 and does not bind to the transport protein vitamin D - binding protein.	bind
35123	1	8501	7	NULL	NULL	0	NULL	 KY3	NULL		bind	NULL	high affinity			VDR	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_102_23_2867_s_24	11104746	6  KY3 has  20 times higher affinity for VDR than 1,25(OH)2D3 and does not bind to the transport protein vitamin D - binding protein.	bind
35124	2	8501	7	NULL	NULL	0	NULL	 1,25(OH)2D3	NULL		bind	NULL				VDR	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_102_23_2867_s_24	11104746	6  KY3 has  20 times higher affinity for VDR than 1,25(OH)2D3 and does not bind to the transport protein vitamin D - binding protein.	bind
35125	3	8501	7	NULL	NULL	0	NULL	statement 1	NULL	affinity of	is higher than	NULL				statement 2	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw60_circulation_102_23_2867_s_24	11104746	6  KY3 has  20 times higher affinity for VDR than 1,25(OH)2D3 and does not bind to the transport protein vitamin D - binding protein.	bind
35126	4	8501	7	NULL	NULL	0	NULL	KY3 	NULL		does not bind	NULL				vitamin D - binding protein	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_102_23_2867_s_24	11104746	6  KY3 has  20 times higher affinity for VDR than 1,25(OH)2D3 and does not bind to the transport protein vitamin D - binding protein.	bind
35127	5	8501	7	NULL	NULL	0	NULL	vitamin D - binding protein	NULL		is a type of	NULL				transport protein	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_102_23_2867_s_24	11104746	6  KY3 has  20 times higher affinity for VDR than 1,25(OH)2D3 and does not bind to the transport protein vitamin D - binding protein.	bind
33568	1	8502	5	13	NULL	NULL	NULL	PlGF	GP		is					placenta growth factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_993_s_22	11549592	6  lacenta growth factor (PlGF) that binds to VEGFR-1 and not VEGFR-2 also stimulates monocyte migration.	bind
33569	2	8502	5	13	NULL	NULL	NULL	PlGF	GP		bind					VEGFR-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_993_s_22	11549592	6  lacenta growth factor (PlGF) that binds to VEGFR-1 and not VEGFR-2 also stimulates monocyte migration.	bind
33570	3	8502	5	13	NULL	NULL	NULL	PlGF	GP		bind					VEGFR-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_993_s_22	11549592	6  lacenta growth factor (PlGF) that binds to VEGFR-1 and not VEGFR-2 also stimulates monocyte migration.	bind
33571	4	8502	5	13	NULL	NULL	NULL	PlGF	GP		stimulates					monocyte	Cell	migration of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_993_s_22	11549592	6  lacenta growth factor (PlGF) that binds to VEGFR-1 and not VEGFR-2 also stimulates monocyte migration.	bind
35128	1	8502	7	NULL	NULL	0	NULL	PlGF	NULL		binds to	NULL				VEGFR-1	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_3_993_s_22	11549592	6  lacenta growth factor (PlGF) that binds to VEGFR-1 and not VEGFR-2 also stimulates monocyte migration.	bind
35129	2	8502	7	NULL	NULL	0	NULL	PlGF	NULL		does not bind	NULL				VEGFR-2	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_3_993_s_22	11549592	6  lacenta growth factor (PlGF) that binds to VEGFR-1 and not VEGFR-2 also stimulates monocyte migration.	bind
35130	3	8502	7	NULL	NULL	0	NULL	PIGF	NULL		stimulates	NULL				monocyte	NULL	migration of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_3_993_s_22	11549592	6  lacenta growth factor (PlGF) that binds to VEGFR-1 and not VEGFR-2 also stimulates monocyte migration.	bind
35131	4	8502	7	NULL	NULL	0	NULL	PlGF	NULL		is	NULL				placenta growth factor 	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_3_993_s_22	11549592	6  lacenta growth factor (PlGF) that binds to VEGFR-1 and not VEGFR-2 also stimulates monocyte migration.	bind
33573	1	8503	5	13	NULL	NULL	NULL	lectin	GP		bind					galactose residues	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_3_1055_s_170	10702421	6  Microglia could not be visualized with the GS lectin in mice given an intracarotid injection of arabinose, because arabinose interferes with the binding of the lectin to the galactose residues.	bind
33574	2	8503	5	13	NULL	NULL	NULL	arabinose	Chemical		interfere with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_3_1055_s_170	10702421	6  Microglia could not be visualized with the GS lectin in mice given an intracarotid injection of arabinose, because arabinose interferes with the binding of the lectin to the galactose residues.	bind
35132	1	8503	7	NULL	NULL	0	NULL	lectin	NULL		bind	NULL				galactose residues	NULL				NULL	mice	NULL	NULL	NULL	NULL	gw60_amjpathol_156_3_1055_s_170	10702421	6  Microglia could not be visualized with the GS lectin in mice given an intracarotid injection of arabinose, because arabinose interferes with the binding of the lectin to the galactose residues.	bind
35133	2	8503	7	NULL	NULL	0	NULL	 arabinose	NULL		interferes with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_3_1055_s_170	10702421	6  Microglia could not be visualized with the GS lectin in mice given an intracarotid injection of arabinose, because arabinose interferes with the binding of the lectin to the galactose residues.	bind
33575	1	8504	5	13	NULL	NULL	NULL	mdm2	GP		regulates					p53	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_3_977_s_27	10702413	6  p53 activity is regulated by mdm2, which binds to p53, inhibits its transcriptional activity, and targets its degradation.	bind
33576	2	8504	5	13	NULL	NULL	NULL	mdm2	GP		bind					p53	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_3_977_s_27	10702413	6  p53 activity is regulated by mdm2, which binds to p53, inhibits its transcriptional activity, and targets its degradation.	bind
33577	3	8504	5	13	NULL	NULL	NULL	statement 2	Process		inhibits					p53	GP	transcriptional activity of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_3_977_s_27	10702413	6  p53 activity is regulated by mdm2, which binds to p53, inhibits its transcriptional activity, and targets its degradation.	bind
33578	4	8504	5	13	NULL	NULL	NULL	statement 2	Process		targets					p53	GP	degradation of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_3_977_s_27	10702413	6  p53 activity is regulated by mdm2, which binds to p53, inhibits its transcriptional activity, and targets its degradation.	bind
35134	1	8504	7	NULL	NULL	0	NULL	mdm2	NULL		regulates	NULL				p53 	NULL	activity of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_3_977_s_27	10702413	6  p53 activity is regulated by mdm2, which binds to p53, inhibits its transcriptional activity, and targets its degradation.	bind
35135	2	8504	7	NULL	NULL	0	NULL	mdm2	NULL		binds to	NULL				p53	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_3_977_s_27	10702413	6  p53 activity is regulated by mdm2, which binds to p53, inhibits its transcriptional activity, and targets its degradation.	bind
35136	3	8504	7	NULL	NULL	0	NULL	mdm2	NULL		inhibits	NULL				p53	NULL	transcriptional activity of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_3_977_s_27	10702413	6  p53 activity is regulated by mdm2, which binds to p53, inhibits its transcriptional activity, and targets its degradation.	bind
35137	4	8504	7	NULL	NULL	0	NULL	mdm2	NULL		target	NULL				p53	NULL	degradation of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_3_977_s_27	10702413	6  p53 activity is regulated by mdm2, which binds to p53, inhibits its transcriptional activity, and targets its degradation.	bind
33581	1	8505	5	13	NULL	NULL	NULL	apoB	GP		bind					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_10_1719_s_154	7583549	6  Since the radius of the LDL particle may vary considerably and, according to this model, also that of the apoB, 25  the stabilization of the two amino acid clusters may be of importance to maintain the binding affinity of the apoB to the LDL receptor.	bind
35146	1	8505	7	NULL	NULL	0	NULL	apoB 	NULL		bind	NULL				LDL receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_10_1719_s_154	7583549	6  Since the radius of the LDL particle may vary considerably and, according to this model, also that of the apoB, 25  the stabilization of the two amino acid clusters may be of importance to maintain the binding affinity of the apoB to the LDL receptor.	bind
33586	1	8506	5	13	NULL	NULL	NULL	SMCs	Cell		bind					fibronectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_12_1855_s_25	9848876	6  SMCs bind to fibronectin, laminin, collagen I, and collagen IV primarily by means of beta1 integrins.	bind
33587	2	8506	5	13	NULL	NULL	NULL	statement 1	Process		occurs via					beta1 integrins	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_12_1855_s_25	9848876	6  SMCs bind to fibronectin, laminin, collagen I, and collagen IV primarily by means of beta1 integrins.	bind
33588	3	8506	5	13	NULL	NULL	NULL	SMCs	Cell		bind					laminin	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_12_1855_s_25	9848876	6  SMCs bind to fibronectin, laminin, collagen I, and collagen IV primarily by means of beta1 integrins.	bind
33589	4	8506	5	13	NULL	NULL	NULL	statement 3	Process		occurs via					beta1 integrins	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_12_1855_s_25	9848876	6  SMCs bind to fibronectin, laminin, collagen I, and collagen IV primarily by means of beta1 integrins.	bind
33590	5	8506	5	13	NULL	NULL	NULL	SMCs	Cell		bind					collagen I	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_12_1855_s_25	9848876	6  SMCs bind to fibronectin, laminin, collagen I, and collagen IV primarily by means of beta1 integrins.	bind
33591	6	8506	5	13	NULL	NULL	NULL	statement 5	Process		occurs via					beta1 integrins	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_12_1855_s_25	9848876	6  SMCs bind to fibronectin, laminin, collagen I, and collagen IV primarily by means of beta1 integrins.	bind
33592	7	8506	5	13	NULL	NULL	NULL	SMCs	Cell		bind					collagen IV	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_12_1855_s_25	9848876	6  SMCs bind to fibronectin, laminin, collagen I, and collagen IV primarily by means of beta1 integrins.	bind
33593	8	8506	5	13	NULL	NULL	NULL	statement 7	Process		occurs via					beta1 integrins	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_12_1855_s_25	9848876	6  SMCs bind to fibronectin, laminin, collagen I, and collagen IV primarily by means of beta1 integrins.	bind
35148	1	8506	7	NULL	NULL	0	NULL	SMCs	NULL		bind	NULL				fibronectin	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_12_1855_s_25	9848876	6  SMCs bind to fibronectin, laminin, collagen I, and collagen IV primarily by means of beta1 integrins.	bind
35149	2	8506	7	NULL	NULL	0	NULL	SMCs	NULL		bind	NULL				laminin	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_12_1855_s_25	9848876	6  SMCs bind to fibronectin, laminin, collagen I, and collagen IV primarily by means of beta1 integrins.	bind
35150	3	8506	7	NULL	NULL	0	NULL	SMCs	NULL		bind	NULL				collagen I	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_12_1855_s_25	9848876	6  SMCs bind to fibronectin, laminin, collagen I, and collagen IV primarily by means of beta1 integrins.	bind
35151	4	8506	7	NULL	NULL	0	NULL	SMCs	NULL		bind	NULL				collagen IV	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_12_1855_s_25	9848876	6  SMCs bind to fibronectin, laminin, collagen I, and collagen IV primarily by means of beta1 integrins.	bind
35178	5	8506	7	NULL	NULL	0	NULL	statement 1	NULL		occurs via	NULL				beta1 integrins	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_12_1855_s_25	9848876	6  SMCs bind to fibronectin, laminin, collagen I, and collagen IV primarily by means of beta1 integrins.	bind
35179	6	8506	7	NULL	NULL	0	NULL	statement 2	NULL		occurs via	NULL				beta1 integrins	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_12_1855_s_25	9848876	6  SMCs bind to fibronectin, laminin, collagen I, and collagen IV primarily by means of beta1 integrins.	bind
35180	7	8506	7	NULL	NULL	0	NULL	statement 3	NULL		occurs via	NULL				beta1 integrins	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_12_1855_s_25	9848876	6  SMCs bind to fibronectin, laminin, collagen I, and collagen IV primarily by means of beta1 integrins.	bind
35181	8	8506	7	NULL	NULL	0	NULL	statement 4	NULL		occurs via	NULL				beta1 integrins	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_12_1855_s_25	9848876	6  SMCs bind to fibronectin, laminin, collagen I, and collagen IV primarily by means of beta1 integrins.	bind
33594	1	8507	5	13	NULL	NULL	NULL	cell wall	CellComponent	changes in;; thickness of 	results in					vancomycin	Chemical	resistance of			NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_49_2_255_s_19	11815565	6 -  8 It is believed that the reason such changes in cell wall thickness and cross-linking result in vancomycin resistance is that the modified cell wall binds more vancomycin, due to the increased amount of terminal d-alanyl-d-alanine dipeptide.	bind
33595	2	8507	5	13	NULL	NULL	NULL	cell wall	CellComponent	changes in;; thickness of	results in					vancomycin	Chemical	resistance of			NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_49_2_255_s_19	11815565	6 -  8 It is believed that the reason such changes in cell wall thickness and cross-linking result in vancomycin resistance is that the modified cell wall binds more vancomycin, due to the increased amount of terminal d-alanyl-d-alanine dipeptide.	bind
33596	3	8507	5	13	NULL	NULL	NULL	cell wall	CellComponent	modified	bind					vancomycin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_49_2_255_s_19	11815565	6 -  8 It is believed that the reason such changes in cell wall thickness and cross-linking result in vancomycin resistance is that the modified cell wall binds more vancomycin, due to the increased amount of terminal d-alanyl-d-alanine dipeptide.	bind
33597	4	8507	5	13	NULL	NULL	NULL	d-alanyl-d-alanine dipeptide	AminoAcid	increased amount of terminal	results in					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_49_2_255_s_19	11815565	6 -  8 It is believed that the reason such changes in cell wall thickness and cross-linking result in vancomycin resistance is that the modified cell wall binds more vancomycin, due to the increased amount of terminal d-alanyl-d-alanine dipeptide.	bind
33598	5	8507	5	13	NULL	NULL	NULL	statement 3	Process		leads to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_49_2_255_s_19	11815565	6 -  8 It is believed that the reason such changes in cell wall thickness and cross-linking result in vancomycin resistance is that the modified cell wall binds more vancomycin, due to the increased amount of terminal d-alanyl-d-alanine dipeptide.	bind
33599	6	8507	5	13	NULL	NULL	NULL	statement 3	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_49_2_255_s_19	11815565	6 -  8 It is believed that the reason such changes in cell wall thickness and cross-linking result in vancomycin resistance is that the modified cell wall binds more vancomycin, due to the increased amount of terminal d-alanyl-d-alanine dipeptide.	bind
35182	1	8507	7	NULL	NULL	0	NULL	cell wall	NULL	modified	binds	NULL				vancomycin	NULL				NULL		0	NULL	NULL	NULL	gw60_jantimicrobchemoth_49_2_255_s_19	11815565	6 -  8 It is believed that the reason such changes in cell wall thickness and cross-linking result in vancomycin resistance is that the modified cell wall binds more vancomycin, due to the increased amount of terminal d-alanyl-d-alanine dipeptide.	bind
35185	2	8507	7	NULL	NULL	0	NULL	statement 1	NULL		occurs due to	NULL				 d-alanyl-d-alanine dipeptide	NULL		terminal		NULL		0	NULL	NULL	NULL	gw60_jantimicrobchemoth_49_2_255_s_19	11815565	6 -  8 It is believed that the reason such changes in cell wall thickness and cross-linking result in vancomycin resistance is that the modified cell wall binds more vancomycin, due to the increased amount of terminal d-alanyl-d-alanine dipeptide.	bind
46725	3	8507	7	NULL	NULL	0	NULL	cell wall 	NULL	changes in thickness of	result in	NULL				vancomycin	NULL	resistance of			NULL		0	NULL	NULL	NULL	gw60_jantimicrobchemoth_49_2_255_s_19	11815565	6 -  8 It is believed that the reason such changes in cell wall thickness and cross-linking result in vancomycin resistance is that the modified cell wall binds more vancomycin, due to the increased amount of terminal d-alanyl-d-alanine dipeptide.	bind
46726	4	8507	7	NULL	NULL	0	NULL	cross-linking	NULL	changes in	result in	NULL				vancomycin	NULL	resistance of			NULL		0	NULL	NULL	NULL	gw60_jantimicrobchemoth_49_2_255_s_19	11815565	6 -  8 It is believed that the reason such changes in cell wall thickness and cross-linking result in vancomycin resistance is that the modified cell wall binds more vancomycin, due to the increased amount of terminal d-alanyl-d-alanine dipeptide.	bind
46727	5	8507	7	10	NULL	0	NULL	statement 1	NULL		leads to	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_49_2_255_s_19	11815565	6 -  8 It is believed that the reason such changes in cell wall thickness and cross-linking result in vancomycin resistance is that the modified cell wall binds more vancomycin, due to the increased amount of terminal d-alanyl-d-alanine dipeptide.	bind
46728	6	8507	7	10	NULL	0	NULL	statement 1	NULL		leads to	NULL				statement 4	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_49_2_255_s_19	11815565	6 -  8 It is believed that the reason such changes in cell wall thickness and cross-linking result in vancomycin resistance is that the modified cell wall binds more vancomycin, due to the increased amount of terminal d-alanyl-d-alanine dipeptide.	bind
33600	1	8509	5	13	NULL	NULL	NULL	RGD	AminoAcid		is					tripeptide arginine-glycine aspartate	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_4_705_s_23	7641347	6 10 11  Many of the biological effects of OPN appear to be mediated by binding of a tripeptide arginine-glycine aspartate (RGD) sequence to cell-surface integrin receptors.	bind
33601	2	8509	5	13	NULL	NULL	NULL	RGD sequence	AminoAcid		bind					integrin receptors	GP	cell-surface			NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_4_705_s_23	7641347	6 10 11  Many of the biological effects of OPN appear to be mediated by binding of a tripeptide arginine-glycine aspartate (RGD) sequence to cell-surface integrin receptors.	bind
33602	3	8509	5	13	NULL	NULL	NULL	OPN	GP	biological effects of	is mediated by					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_4_705_s_23	7641347	6 10 11  Many of the biological effects of OPN appear to be mediated by binding of a tripeptide arginine-glycine aspartate (RGD) sequence to cell-surface integrin receptors.	bind
35187	1	8509	7	10	NULL	0	NULL	RGD tripeptide			bind					integrin receptors		cell-surface			NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_4_705_s_23	7641347	6 10 11  Many of the biological effects of OPN appear to be mediated by binding of a tripeptide arginine-glycine aspartate (RGD) sequence to cell-surface integrin receptors.	bind
35188	2	8509	7	NULL	NULL	0	NULL	statement 1	NULL		mediates	NULL				OPN	NULL	biological effects of			NULL		0	NULL	NULL	NULL	gw60_circulation_92_4_705_s_23	7641347	6 10 11  Many of the biological effects of OPN appear to be mediated by binding of a tripeptide arginine-glycine aspartate (RGD) sequence to cell-surface integrin receptors.	bind
35189	3	8509	7	NULL	NULL	0	NULL	RGD	NULL		is	NULL				arginine-glycine aspartate	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_4_705_s_23	7641347	6 10 11  Many of the biological effects of OPN appear to be mediated by binding of a tripeptide arginine-glycine aspartate (RGD) sequence to cell-surface integrin receptors.	bind
33603	1	8510	5	13	NULL	NULL	NULL	Wg protein	GP	soluble	bind					fz proteins	GP	Drosophila			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_12_1433_s_30	10381896	6 11 12  The importance of the fz-Wnt interaction was highlighted by the fact that cells transfected with soluble Wg protein bind both  Drosophila and mammalian fz proteins and initiate signal.	bind
33604	2	8510	5	13	NULL	NULL	NULL	statement 1	Process		initiates					signal	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_12_1433_s_30	10381896	6 11 12  The importance of the fz-Wnt interaction was highlighted by the fact that cells transfected with soluble Wg protein bind both  Drosophila and mammalian fz proteins and initiate signal.	bind
33605	3	8510	5	13	NULL	NULL	NULL	Wg protein	GP	soluble	bind					fz proteins	GP	mammalian			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_12_1433_s_30	10381896	6 11 12  The importance of the fz-Wnt interaction was highlighted by the fact that cells transfected with soluble Wg protein bind both  Drosophila and mammalian fz proteins and initiate signal.	bind
33606	4	8510	5	13	NULL	NULL	NULL	statement 3	Process		initiates					signal	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_12_1433_s_30	10381896	6 11 12  The importance of the fz-Wnt interaction was highlighted by the fact that cells transfected with soluble Wg protein bind both  Drosophila and mammalian fz proteins and initiate signal.	bind
35192	1	8510	7	NULL	NULL	0	NULL	 Wg protein	NULL	soluble	bind	NULL				 fz proteins	NULL	Drosophila 			NULL		0	NULL	NULL	NULL	gw60_circulationres_84_12_1433_s_30	10381896	6 11 12  The importance of the fz-Wnt interaction was highlighted by the fact that cells transfected with soluble Wg protein bind both  Drosophila and mammalian fz proteins and initiate signal.	bind
35193	2	8510	7	NULL	NULL	0	NULL	Wg protein	NULL	soluble	bind	NULL				fz proteins	NULL	mammalian			NULL		0	NULL	NULL	NULL	gw60_circulationres_84_12_1433_s_30	10381896	6 11 12  The importance of the fz-Wnt interaction was highlighted by the fact that cells transfected with soluble Wg protein bind both  Drosophila and mammalian fz proteins and initiate signal.	bind
35196	3	8510	7	NULL	NULL	0	NULL	statement 1	NULL		initiate	NULL				signal	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_12_1433_s_30	10381896	6 11 12  The importance of the fz-Wnt interaction was highlighted by the fact that cells transfected with soluble Wg protein bind both  Drosophila and mammalian fz proteins and initiate signal.	bind
35197	4	8510	7	NULL	NULL	0	NULL	statement 2	NULL		initiate	NULL				signal	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_12_1433_s_30	10381896	6 11 12  The importance of the fz-Wnt interaction was highlighted by the fact that cells transfected with soluble Wg protein bind both  Drosophila and mammalian fz proteins and initiate signal.	bind
33607	1	8511	5	13	NULL	NULL	NULL	apoB	GP	defective	bind					LDLR	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_10_1719_s_210	7583549	6 25 26  Since the size of the LDL particles has been demonstrated to be of importance for the binding of the defective apoB to the LDLR, 6  dietary changes may therefore cause a change in the binding affinity of the apoB.	bind
33609	2	8511	5	13	NULL	NULL	NULL	dietary changes			change		may			apoB	GP	binding affinity of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_10_1719_s_210	7583549	6 25 26  Since the size of the LDL particles has been demonstrated to be of importance for the binding of the defective apoB to the LDLR, 6  dietary changes may therefore cause a change in the binding affinity of the apoB.	bind
35200	1	8511	7	10	NULL	0	NULL	apoB		defective 	bind					LDLR					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_10_1719_s_210	7583549	6 25 26  Since the size of the LDL particles has been demonstrated to be of importance for the binding of the defective apoB to the LDLR, 6  dietary changes may therefore cause a change in the binding affinity of the apoB.	bind
35201	2	8511	7	NULL	NULL	0	NULL	dietary changes	NULL		change	NULL	may			apoB	NULL	binding affinity of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_10_1719_s_210	7583549	6 25 26  Since the size of the LDL particles has been demonstrated to be of importance for the binding of the defective apoB to the LDLR, 6  dietary changes may therefore cause a change in the binding affinity of the apoB.	bind
33615	1	8512	5	13	NULL	NULL	NULL	VLDLR	GP		bind					beta-VLDL	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_3_407_s_23	8630667	6 7  LRP, like the VLDLR, also binds beta-VLDL; however, unlike the VLDLR, LRP binds beta-VLDL only when the latter particle has been supplemented with exogenous apoE. 1 8	bind
33616	2	8512	5	13	NULL	NULL	NULL	LRP	GP		bind					beta-VLDL	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_3_407_s_23	8630667	6 7  LRP, like the VLDLR, also binds beta-VLDL; however, unlike the VLDLR, LRP binds beta-VLDL only when the latter particle has been supplemented with exogenous apoE. 1 8	bind
33617	3	8512	5	13	NULL	NULL	NULL	beta-VLDL	GP		is supplemented with					apoE	GP	exogenous			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_3_407_s_23	8630667	6 7  LRP, like the VLDLR, also binds beta-VLDL; however, unlike the VLDLR, LRP binds beta-VLDL only when the latter particle has been supplemented with exogenous apoE. 1 8	bind
33618	4	8512	5	13	NULL	NULL	NULL	statement 2	Process		occurs following		only			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_3_407_s_23	8630667	6 7  LRP, like the VLDLR, also binds beta-VLDL; however, unlike the VLDLR, LRP binds beta-VLDL only when the latter particle has been supplemented with exogenous apoE. 1 8	bind
35202	1	8512	7	NULL	NULL	0	NULL	LRP	NULL		binds	NULL				beta-VLDL	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_3_407_s_23	8630667	6 7  LRP, like the VLDLR, also binds beta-VLDL; however, unlike the VLDLR, LRP binds beta-VLDL only when the latter particle has been supplemented with exogenous apoE. 1 8	bind
35203	2	8512	7	NULL	NULL	0	NULL	VLDLR	NULL		binds	NULL				beta-VLDL	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_3_407_s_23	8630667	6 7  LRP, like the VLDLR, also binds beta-VLDL; however, unlike the VLDLR, LRP binds beta-VLDL only when the latter particle has been supplemented with exogenous apoE. 1 8	bind
35204	3	8512	7	10	NULL	0	NULL	beta-VLDL			is supplemented with					apoE		exogenous 			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_3_407_s_23	8630667	6 7  LRP, like the VLDLR, also binds beta-VLDL; however, unlike the VLDLR, LRP binds beta-VLDL only when the latter particle has been supplemented with exogenous apoE. 1 8	bind
55799	4	8512	7	10	NULL	0	NULL	statement 2			occurs following		only			statement 3					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_3_407_s_23	8630667	6 7  LRP, like the VLDLR, also binds beta-VLDL; however, unlike the VLDLR, LRP binds beta-VLDL only when the latter particle has been supplemented with exogenous apoE. 1 8	bind
33610	1	8513	5	13	NULL	NULL	NULL	LDL particles	GP		bind					LDL B receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1573_s_159	8977464	6 7  Oxidation of LDL particles impairs their binding to LDL B,E receptors and thus confines their uptake mainly by macrophages via the scavenger receptor pathway.	bind
33611	2	8513	5	13	NULL	NULL	NULL	LDL particles	GP	oxidation of	impairs					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1573_s_159	8977464	6 7  Oxidation of LDL particles impairs their binding to LDL B,E receptors and thus confines their uptake mainly by macrophages via the scavenger receptor pathway.	bind
33613	4	8513	5	13	NULL	NULL	NULL	statement 2	Process		confines					macrophages	Cell	uptake by			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1573_s_159	8977464	6 7  Oxidation of LDL particles impairs their binding to LDL B,E receptors and thus confines their uptake mainly by macrophages via the scavenger receptor pathway.	bind
33614	5	8513	5	13	NULL	NULL	NULL	statement 4	Process		via					scavenger receptor pathway	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1573_s_159	8977464	6 7  Oxidation of LDL particles impairs their binding to LDL B,E receptors and thus confines their uptake mainly by macrophages via the scavenger receptor pathway.	bind
56464	3	8513	5	13	NULL	NULL	NULL	LDL particles	GP		bind					LDL E receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1573_s_159	8977464	6 7  Oxidation of LDL particles impairs their binding to LDL B,E receptors and thus confines their uptake mainly by macrophages via the scavenger receptor pathway.	bind
56465	6	8513	5	13	NULL	NULL	NULL	statement 3	Process		confines					macrophages	Cell	uptake by			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1573_s_159	8977464	6 7  Oxidation of LDL particles impairs their binding to LDL B,E receptors and thus confines their uptake mainly by macrophages via the scavenger receptor pathway.	bind
56466	7	8513	5	13	NULL	NULL	NULL	statement 6	Process		via					scavenger receptor pathway	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1573_s_159	8977464	6 7  Oxidation of LDL particles impairs their binding to LDL B,E receptors and thus confines their uptake mainly by macrophages via the scavenger receptor pathway.	bind
56467	8	8513	5	13	NULL	NULL	NULL	LDL particles	GP	oxidation of	impairs					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1573_s_159	8977464	6 7  Oxidation of LDL particles impairs their binding to LDL B,E receptors and thus confines their uptake mainly by macrophages via the scavenger receptor pathway.	bind
35206	1	8513	7	NULL	NULL	0	NULL	 LDL particles	NULL		bind	NULL				LDL B receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1573_s_159	8977464	6 7  Oxidation of LDL particles impairs their binding to LDL B,E receptors and thus confines their uptake mainly by macrophages via the scavenger receptor pathway.	bind
35207	2	8513	7	NULL	NULL	0	NULL	LDL particles	NULL		bind	NULL				LDL E receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1573_s_159	8977464	6 7  Oxidation of LDL particles impairs their binding to LDL B,E receptors and thus confines their uptake mainly by macrophages via the scavenger receptor pathway.	bind
35208	3	8513	7	NULL	NULL	0	NULL	LDL particles	NULL	oxidation of	impair	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1573_s_159	8977464	6 7  Oxidation of LDL particles impairs their binding to LDL B,E receptors and thus confines their uptake mainly by macrophages via the scavenger receptor pathway.	bind
35209	4	8513	7	NULL	NULL	0	NULL	LDL particles	NULL	oxidation of	impair	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1573_s_159	8977464	6 7  Oxidation of LDL particles impairs their binding to LDL B,E receptors and thus confines their uptake mainly by macrophages via the scavenger receptor pathway.	bind
35210	5	8513	7	NULL	NULL	0	NULL	statement 1	NULL		confines	NULL				macrophages	NULL	uptake by			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1573_s_159	8977464	6 7  Oxidation of LDL particles impairs their binding to LDL B,E receptors and thus confines their uptake mainly by macrophages via the scavenger receptor pathway.	bind
35211	6	8513	7	NULL	NULL	0	NULL	statement 2	NULL		confines	NULL				macrophages	NULL	uptake by			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1573_s_159	8977464	6 7  Oxidation of LDL particles impairs their binding to LDL B,E receptors and thus confines their uptake mainly by macrophages via the scavenger receptor pathway.	bind
35219	7	8513	7	NULL	NULL	0	NULL	statement 5	NULL		occurs via	NULL				scavenger receptor pathway	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1573_s_159	8977464	6 7  Oxidation of LDL particles impairs their binding to LDL B,E receptors and thus confines their uptake mainly by macrophages via the scavenger receptor pathway.	bind
35220	8	8513	7	NULL	NULL	0	NULL	statement 6	NULL		occurs via	NULL				scavenger receptor pathway	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_12_1573_s_159	8977464	6 7  Oxidation of LDL particles impairs their binding to LDL B,E receptors and thus confines their uptake mainly by macrophages via the scavenger receptor pathway.	bind
46667	1	8514	5	13	NULL	NULL	NULL	[3]SCH58261	Chemical		bind		specifically			crude membranes	CellComponent				NULL	porcine striatum	NULL	NULL	NULL	NULL	gw60_circulationres_79_6_1153_s_194	8943953	6 7  The specific binding of [3]SCH58261 to crude membranes prepared from porcine striatum and PC12 cells was 85% and 90% of total binding at the  Kd value, respectively, whereas the specific binding of [3]KF 178375 and [125]ZM 241385 to membranes prepared from rat and bovine striatum was 60% to 70% of total binding.	bind
46668	2	8514	5	13	NULL	NULL	NULL	[3]SCH58261	Chemical		bind		specifically			crude membranes	CellComponent				NULL	PC12 cells	NULL	NULL	NULL	NULL	gw60_circulationres_79_6_1153_s_194	8943953	6 7  The specific binding of [3]SCH58261 to crude membranes prepared from porcine striatum and PC12 cells was 85% and 90% of total binding at the  Kd value, respectively, whereas the specific binding of [3]KF 178375 and [125]ZM 241385 to membranes prepared from rat and bovine striatum was 60% to 70% of total binding.	bind
46669	3	8514	5	13	NULL	NULL	NULL	[3]KF 178375	Chemical		bind		specifically			membranes	CellComponent				NULL	rat striatum	NULL	NULL	NULL	NULL	gw60_circulationres_79_6_1153_s_194	8943953	6 7  The specific binding of [3]SCH58261 to crude membranes prepared from porcine striatum and PC12 cells was 85% and 90% of total binding at the  Kd value, respectively, whereas the specific binding of [3]KF 178375 and [125]ZM 241385 to membranes prepared from rat and bovine striatum was 60% to 70% of total binding.	bind
46672	4	8514	5	13	NULL	NULL	NULL	[125]ZM 241385	Chemical		bind		specifically			membrane	CellComponent				NULL	bovine striatum	NULL	NULL	NULL	NULL	gw60_circulationres_79_6_1153_s_194	8943953	6 7  The specific binding of [3]SCH58261 to crude membranes prepared from porcine striatum and PC12 cells was 85% and 90% of total binding at the  Kd value, respectively, whereas the specific binding of [3]KF 178375 and [125]ZM 241385 to membranes prepared from rat and bovine striatum was 60% to 70% of total binding.	bind
35221	1	8514	7	NULL	NULL	0	NULL	[3]SCH58261	NULL		bind	NULL	specifically			crude membranes	NULL				NULL	porcine striatum	0	NULL	NULL	NULL	gw60_circulationres_79_6_1153_s_194	8943953	6 7  The specific binding of [3]SCH58261 to crude membranes prepared from porcine striatum and PC12 cells was 85% and 90% of total binding at the  Kd value, respectively, whereas the specific binding of [3]KF 178375 and [125]ZM 241385 to membranes prepared from rat and bovine striatum was 60% to 70% of total binding.	bind
35222	2	8514	7	NULL	NULL	0	NULL	[3]SCH58261	NULL		bind	NULL	specifically			crude membranes	NULL				NULL	PC12 cells	NULL	NULL	NULL	NULL	gw60_circulationres_79_6_1153_s_194	8943953	6 7  The specific binding of [3]SCH58261 to crude membranes prepared from porcine striatum and PC12 cells was 85% and 90% of total binding at the  Kd value, respectively, whereas the specific binding of [3]KF 178375 and [125]ZM 241385 to membranes prepared from rat and bovine striatum was 60% to 70% of total binding.	bind
35223	3	8514	7	NULL	NULL	0	NULL	[3]KF 178375	NULL		bind	NULL	specifically			membranes	NULL				NULL	rat striatum	0	NULL	NULL	NULL	gw60_circulationres_79_6_1153_s_194	8943953	6 7  The specific binding of [3]SCH58261 to crude membranes prepared from porcine striatum and PC12 cells was 85% and 90% of total binding at the  Kd value, respectively, whereas the specific binding of [3]KF 178375 and [125]ZM 241385 to membranes prepared from rat and bovine striatum was 60% to 70% of total binding.	bind
35224	4	8514	7	NULL	NULL	0	NULL	 [125]ZM 241385	NULL		bind	NULL	specifically			membranes	NULL				NULL	bovine striatum	NULL	NULL	NULL	NULL	gw60_circulationres_79_6_1153_s_194	8943953	6 7  The specific binding of [3]SCH58261 to crude membranes prepared from porcine striatum and PC12 cells was 85% and 90% of total binding at the  Kd value, respectively, whereas the specific binding of [3]KF 178375 and [125]ZM 241385 to membranes prepared from rat and bovine striatum was 60% to 70% of total binding.	bind
33625	1	8515	5	13	NULL	NULL	NULL	plasminogen	GP		bind					lysine	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_5_656_s_24	8963723	6 7  This activity is responsible for the binding of plasminogen to lysine-Sepharose and, more importantly, for the interaction of plasminogen and plasmin with substrates, 8 9  inhibitors, 10  and cellular receptors.	bind
35229	1	8515	7	10	NULL	0	NULL	plasminogen			bind					lysine					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_5_656_s_24	8963723	6 7  This activity is responsible for the binding of plasminogen to lysine-Sepharose and, more importantly, for the interaction of plasminogen and plasmin with substrates, 8 9  inhibitors, 10  and cellular receptors.	bind
33639	1	8516	5	13	NULL	NULL	NULL	FKBP12	GP		bind					RyR1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_2_188_s_29	11157671	6 7 8 9  Although FKBP12 can bind to both RyR1 and RyR2, FKBP12.6 specifically associates with RyR2.	bind
33640	2	8516	5	13	NULL	NULL	NULL	FKBP12	GP		bind					RyR2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_2_188_s_29	11157671	6 7 8 9  Although FKBP12 can bind to both RyR1 and RyR2, FKBP12.6 specifically associates with RyR2.	bind
33641	3	8516	5	13	NULL	NULL	NULL	FKBP12.6	GP		associates with		specifically			RyR2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_2_188_s_29	11157671	6 7 8 9  Although FKBP12 can bind to both RyR1 and RyR2, FKBP12.6 specifically associates with RyR2.	bind
35237	1	8516	7	NULL	NULL	0	NULL	FKBP12	NULL		bind	NULL				RyR1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_88_2_188_s_29	11157671	6 7 8 9  Although FKBP12 can bind to both RyR1 and RyR2, FKBP12.6 specifically associates with RyR2.	bind
35238	2	8516	7	NULL	NULL	0	NULL	FKBP12	NULL		bind	NULL				RyR2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_88_2_188_s_29	11157671	6 7 8 9  Although FKBP12 can bind to both RyR1 and RyR2, FKBP12.6 specifically associates with RyR2.	bind
35239	3	8516	7	NULL	NULL	0	NULL	FKBP12.6	NULL		associate with	NULL	specifically			RyR2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_88_2_188_s_29	11157671	6 7 8 9  Although FKBP12 can bind to both RyR1 and RyR2, FKBP12.6 specifically associates with RyR2.	bind
33642	1	8517	5	13	NULL	NULL	NULL	myosin	GP		interacts with					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_11_1310_s_177	10364569	6 7 8 9  In addition, as there appear to be differences in this reciprocal coupling process dependent on whether the myosin interaction with actin is noncycling (rigor) or cycling, 8  it seems possible that crossbridges with different inherent rates of cycling may also differentially affect the activation of the thin filament.	bind
33643	2	8517	5	13	NULL	NULL	NULL	statement 1	Process		is					noncycling	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_11_1310_s_177	10364569	6 7 8 9  In addition, as there appear to be differences in this reciprocal coupling process dependent on whether the myosin interaction with actin is noncycling (rigor) or cycling, 8  it seems possible that crossbridges with different inherent rates of cycling may also differentially affect the activation of the thin filament.	bind
46661	3	8517	5	13	NULL	NULL	NULL	statement 1	Process		is					cycling	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_11_1310_s_177	10364569	6 7 8 9  In addition, as there appear to be differences in this reciprocal coupling process dependent on whether the myosin interaction with actin is noncycling (rigor) or cycling, 8  it seems possible that crossbridges with different inherent rates of cycling may also differentially affect the activation of the thin filament.	bind
46662	4	8517	5	13	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_11_1310_s_177	10364569	6 7 8 9  In addition, as there appear to be differences in this reciprocal coupling process dependent on whether the myosin interaction with actin is noncycling (rigor) or cycling, 8  it seems possible that crossbridges with different inherent rates of cycling may also differentially affect the activation of the thin filament.	bind
46663	5	8517	5	13	NULL	NULL	NULL	statement 2	Process		affects					thin filament	CellComponent	activation of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_11_1310_s_177	10364569	6 7 8 9  In addition, as there appear to be differences in this reciprocal coupling process dependent on whether the myosin interaction with actin is noncycling (rigor) or cycling, 8  it seems possible that crossbridges with different inherent rates of cycling may also differentially affect the activation of the thin filament.	bind
46664	6	8517	5	13	NULL	NULL	NULL	statement 3	Process		affects					thin filament	CellComponent	activation of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_11_1310_s_177	10364569	6 7 8 9  In addition, as there appear to be differences in this reciprocal coupling process dependent on whether the myosin interaction with actin is noncycling (rigor) or cycling, 8  it seems possible that crossbridges with different inherent rates of cycling may also differentially affect the activation of the thin filament.	bind
35240	1	8517	7	NULL	NULL	0	NULL	myosin	NULL		interacts with	NULL				actin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_11_1310_s_177	10364569	6 7 8 9  In addition, as there appear to be differences in this reciprocal coupling process dependent on whether the myosin interaction with actin is noncycling (rigor) or cycling, 8  it seems possible that crossbridges with different inherent rates of cycling may also differentially affect the activation of the thin filament.	bind
35241	2	8517	7	NULL	NULL	0	NULL	statement 1	NULL		is	NULL				noncycling	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_11_1310_s_177	10364569	6 7 8 9  In addition, as there appear to be differences in this reciprocal coupling process dependent on whether the myosin interaction with actin is noncycling (rigor) or cycling, 8  it seems possible that crossbridges with different inherent rates of cycling may also differentially affect the activation of the thin filament.	bind
35242	3	8517	7	NULL	NULL	0	NULL	statement 1	NULL		is	NULL				cycling	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_11_1310_s_177	10364569	6 7 8 9  In addition, as there appear to be differences in this reciprocal coupling process dependent on whether the myosin interaction with actin is noncycling (rigor) or cycling, 8  it seems possible that crossbridges with different inherent rates of cycling may also differentially affect the activation of the thin filament.	bind
35243	4	8517	7	NULL	NULL	0	NULL	statement 2	NULL		is an alternative to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_11_1310_s_177	10364569	6 7 8 9  In addition, as there appear to be differences in this reciprocal coupling process dependent on whether the myosin interaction with actin is noncycling (rigor) or cycling, 8  it seems possible that crossbridges with different inherent rates of cycling may also differentially affect the activation of the thin filament.	bind
35244	5	8517	7	NULL	NULL	0	NULL	statement 2	NULL		affect	NULL				thin filament	NULL	activation of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_11_1310_s_177	10364569	6 7 8 9  In addition, as there appear to be differences in this reciprocal coupling process dependent on whether the myosin interaction with actin is noncycling (rigor) or cycling, 8  it seems possible that crossbridges with different inherent rates of cycling may also differentially affect the activation of the thin filament.	bind
35245	6	8517	7	NULL	NULL	0	NULL	statement 3	NULL		affect	NULL				thin filament	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_circulationres_84_11_1310_s_177	10364569	6 7 8 9  In addition, as there appear to be differences in this reciprocal coupling process dependent on whether the myosin interaction with actin is noncycling (rigor) or cycling, 8  it seems possible that crossbridges with different inherent rates of cycling may also differentially affect the activation of the thin filament.	bind
33644	1	8518	5	13	NULL	NULL	NULL	VEGF-A isoforms	GP		bind					VEGFR-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1578_s_52	15231518	6 All VEGF-A isoforms bind to VEGFR-1 and VEGFR-2.	bind
33645	2	8518	5	13	NULL	NULL	NULL	VEGF-A isoforms	GP		bind					VEGFR-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1578_s_52	15231518	6 All VEGF-A isoforms bind to VEGFR-1 and VEGFR-2.	bind
35246	1	8518	7	NULL	NULL	0	NULL	VEGF-A isoform	NULL		bind	NULL				VEGFR-1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1578_s_52	15231518	6 All VEGF-A isoforms bind to VEGFR-1 and VEGFR-2.	bind
35247	2	8518	7	NULL	NULL	0	NULL	VEGF-A isoforms	NULL		bind	NULL				VEGFR-2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1578_s_52	15231518	6 All VEGF-A isoforms bind to VEGFR-1 and VEGFR-2.	bind
33829	1	8519	5	13	NULL	NULL	NULL	Ang1	GP		bind					Tie2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_8_1014_s_45	16645151	6 Ang1 and Ang2 bind to Tie2 with similar affinities; however, whereas Ang1 is an agonist, the ability of Ang2 to activate Tie2 appears to depend on the cell type and context.	bind
33830	2	8519	5	13	NULL	NULL	NULL	Ang2	GP		bind					Tie2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_8_1014_s_45	16645151	6 Ang1 and Ang2 bind to Tie2 with similar affinities; however, whereas Ang1 is an agonist, the ability of Ang2 to activate Tie2 appears to depend on the cell type and context.	bind
33831	3	8519	5	13	NULL	NULL	NULL	statement 1	Process		similar affinity to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_8_1014_s_45	16645151	6 Ang1 and Ang2 bind to Tie2 with similar affinities; however, whereas Ang1 is an agonist, the ability of Ang2 to activate Tie2 appears to depend on the cell type and context.	bind
33832	4	8519	5	13	NULL	NULL	NULL	Ang1	GP		is agonist of					Tie2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_8_1014_s_45	16645151	6 Ang1 and Ang2 bind to Tie2 with similar affinities; however, whereas Ang1 is an agonist, the ability of Ang2 to activate Tie2 appears to depend on the cell type and context.	bind
33833	5	8519	5	13	NULL	NULL	NULL	Ang2	GP		activates					Tie2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_8_1014_s_45	16645151	6 Ang1 and Ang2 bind to Tie2 with similar affinities; however, whereas Ang1 is an agonist, the ability of Ang2 to activate Tie2 appears to depend on the cell type and context.	bind
33834	6	8519	5	13	NULL	NULL	NULL	statement 5	Process		depends on		may			cell type	Cell				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_8_1014_s_45	16645151	6 Ang1 and Ang2 bind to Tie2 with similar affinities; however, whereas Ang1 is an agonist, the ability of Ang2 to activate Tie2 appears to depend on the cell type and context.	bind
33835	7	8519	5	13	NULL	NULL	NULL	statement 5	Process		depends on		may			context					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_8_1014_s_45	16645151	6 Ang1 and Ang2 bind to Tie2 with similar affinities; however, whereas Ang1 is an agonist, the ability of Ang2 to activate Tie2 appears to depend on the cell type and context.	bind
35248	1	8519	7	NULL	NULL	0	NULL	Ang1	NULL		binds to	NULL				Tie2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_8_1014_s_45	16645151	6 Ang1 and Ang2 bind to Tie2 with similar affinities; however, whereas Ang1 is an agonist, the ability of Ang2 to activate Tie2 appears to depend on the cell type and context.	bind
35249	2	8519	7	NULL	NULL	0	NULL	Ang2	NULL		binds to	NULL				Tie2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_8_1014_s_45	16645151	6 Ang1 and Ang2 bind to Tie2 with similar affinities; however, whereas Ang1 is an agonist, the ability of Ang2 to activate Tie2 appears to depend on the cell type and context.	bind
35250	3	8519	7	NULL	NULL	0	NULL	statement 1	NULL	affinity of	is similar to	NULL				statement 2	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw70_circulationres_98_8_1014_s_45	16645151	6 Ang1 and Ang2 bind to Tie2 with similar affinities; however, whereas Ang1 is an agonist, the ability of Ang2 to activate Tie2 appears to depend on the cell type and context.	bind
35251	4	8519	7	NULL	NULL	0	NULL	Ang1	NULL		is a type of	NULL				agonist	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_8_1014_s_45	16645151	6 Ang1 and Ang2 bind to Tie2 with similar affinities; however, whereas Ang1 is an agonist, the ability of Ang2 to activate Tie2 appears to depend on the cell type and context.	bind
35252	5	8519	7	NULL	NULL	0	NULL	Ang2	NULL		activate	NULL				Tie2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_8_1014_s_45	16645151	6 Ang1 and Ang2 bind to Tie2 with similar affinities; however, whereas Ang1 is an agonist, the ability of Ang2 to activate Tie2 appears to depend on the cell type and context.	bind
35253	6	8519	7	10	NULL	0	NULL	statement 5			depend on		may			cell type					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_8_1014_s_45	16645151	6 Ang1 and Ang2 bind to Tie2 with similar affinities; however, whereas Ang1 is an agonist, the ability of Ang2 to activate Tie2 appears to depend on the cell type and context.	bind
35254	7	8519	7	10	NULL	0	NULL	statement 5			depend on		may			cell context					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_8_1014_s_45	16645151	6 Ang1 and Ang2 bind to Tie2 with similar affinities; however, whereas Ang1 is an agonist, the ability of Ang2 to activate Tie2 appears to depend on the cell type and context.	bind
33646	1	8520	5	13	NULL	NULL	NULL	VLDL	GP	apoE-rich	bind					LDL receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_146	11557678	6 ApoC-III reduces the binding of apoE-rich VLDL to LDL receptors, 26 the LDL receptor - related protein, 8 and proteoglycan 11, 27 and inhibits VLDL uptake by the liver, 28 antagonizing the accelerating effect of apoE on particle clearance.	bind
33647	2	8520	5	13	NULL	NULL	NULL	ApoC-III	GP		reduces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_146	11557678	6 ApoC-III reduces the binding of apoE-rich VLDL to LDL receptors, 26 the LDL receptor - related protein, 8 and proteoglycan 11, 27 and inhibits VLDL uptake by the liver, 28 antagonizing the accelerating effect of apoE on particle clearance.	bind
33648	3	8520	5	13	NULL	NULL	NULL	VLDL	GP	apoE-rich	bind					LDL receptor - related protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_146	11557678	6 ApoC-III reduces the binding of apoE-rich VLDL to LDL receptors, 26 the LDL receptor - related protein, 8 and proteoglycan 11, 27 and inhibits VLDL uptake by the liver, 28 antagonizing the accelerating effect of apoE on particle clearance.	bind
33649	4	8520	5	13	NULL	NULL	NULL	ApoC-III	GP		reduces					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_146	11557678	6 ApoC-III reduces the binding of apoE-rich VLDL to LDL receptors, 26 the LDL receptor - related protein, 8 and proteoglycan 11, 27 and inhibits VLDL uptake by the liver, 28 antagonizing the accelerating effect of apoE on particle clearance.	bind
33650	5	8520	5	13	NULL	NULL	NULL	VLDL	GP	apoE-rich	bind					proteoglycan	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_146	11557678	6 ApoC-III reduces the binding of apoE-rich VLDL to LDL receptors, 26 the LDL receptor - related protein, 8 and proteoglycan 11, 27 and inhibits VLDL uptake by the liver, 28 antagonizing the accelerating effect of apoE on particle clearance.	bind
33651	6	8520	5	13	NULL	NULL	NULL	ApoC-III	GP		reduces					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_146	11557678	6 ApoC-III reduces the binding of apoE-rich VLDL to LDL receptors, 26 the LDL receptor - related protein, 8 and proteoglycan 11, 27 and inhibits VLDL uptake by the liver, 28 antagonizing the accelerating effect of apoE on particle clearance.	bind
33652	7	8520	5	13	NULL	NULL	NULL	VLDL	GP		uptake by					liver	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_146	11557678	6 ApoC-III reduces the binding of apoE-rich VLDL to LDL receptors, 26 the LDL receptor - related protein, 8 and proteoglycan 11, 27 and inhibits VLDL uptake by the liver, 28 antagonizing the accelerating effect of apoE on particle clearance.	bind
33653	8	8520	5	13	NULL	NULL	NULL	apoE 	GP		accelerates					particle clearance	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_146	11557678	6 ApoC-III reduces the binding of apoE-rich VLDL to LDL receptors, 26 the LDL receptor - related protein, 8 and proteoglycan 11, 27 and inhibits VLDL uptake by the liver, 28 antagonizing the accelerating effect of apoE on particle clearance.	bind
33654	9	8520	5	13	NULL	NULL	NULL	statement 7	Process		antagonize					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_146	11557678	6 ApoC-III reduces the binding of apoE-rich VLDL to LDL receptors, 26 the LDL receptor - related protein, 8 and proteoglycan 11, 27 and inhibits VLDL uptake by the liver, 28 antagonizing the accelerating effect of apoE on particle clearance.	bind
55800	10	8520	5	13	NULL	NULL	NULL	ApoC-III	GP		inhibits					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_146	11557678	6 ApoC-III reduces the binding of apoE-rich VLDL to LDL receptors, 26 the LDL receptor - related protein, 8 and proteoglycan 11, 27 and inhibits VLDL uptake by the liver, 28 antagonizing the accelerating effect of apoE on particle clearance.	bind
35255	1	8520	7	10	NULL	0	NULL	VLDL	NULL	 apoE-rich 	bind	NULL				LDL receptor	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_146	11557678	6 ApoC-III reduces the binding of apoE-rich VLDL to LDL receptors, 26 the LDL receptor - related protein, 8 and proteoglycan 11, 27 and inhibits VLDL uptake by the liver, 28 antagonizing the accelerating effect of apoE on particle clearance.	bind
35256	2	8520	7	10	NULL	0	NULL	VLDL	NULL	apoE-rich	bind	NULL				LDL receptor - related protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_146	11557678	6 ApoC-III reduces the binding of apoE-rich VLDL to LDL receptors, 26 the LDL receptor - related protein, 8 and proteoglycan 11, 27 and inhibits VLDL uptake by the liver, 28 antagonizing the accelerating effect of apoE on particle clearance.	bind
35257	3	8520	7	10	NULL	0	NULL	VLDL	NULL	apoE-rich 	bind	NULL				proteoglycan	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_146	11557678	6 ApoC-III reduces the binding of apoE-rich VLDL to LDL receptors, 26 the LDL receptor - related protein, 8 and proteoglycan 11, 27 and inhibits VLDL uptake by the liver, 28 antagonizing the accelerating effect of apoE on particle clearance.	bind
35258	4	8520	7	NULL	NULL	0	NULL	ApoC-III 	NULL		reduce	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_146	11557678	6 ApoC-III reduces the binding of apoE-rich VLDL to LDL receptors, 26 the LDL receptor - related protein, 8 and proteoglycan 11, 27 and inhibits VLDL uptake by the liver, 28 antagonizing the accelerating effect of apoE on particle clearance.	bind
35260	5	8520	7	NULL	NULL	0	NULL	ApoC-III 	NULL		reduce	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_146	11557678	6 ApoC-III reduces the binding of apoE-rich VLDL to LDL receptors, 26 the LDL receptor - related protein, 8 and proteoglycan 11, 27 and inhibits VLDL uptake by the liver, 28 antagonizing the accelerating effect of apoE on particle clearance.	bind
35262	6	8520	7	NULL	NULL	0	NULL	ApoC-III 	NULL		reduce	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_146	11557678	6 ApoC-III reduces the binding of apoE-rich VLDL to LDL receptors, 26 the LDL receptor - related protein, 8 and proteoglycan 11, 27 and inhibits VLDL uptake by the liver, 28 antagonizing the accelerating effect of apoE on particle clearance.	bind
35264	7	8520	7	NULL	NULL	0	NULL	VLDL	NULL		uptake by	NULL				liver	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_146	11557678	6 ApoC-III reduces the binding of apoE-rich VLDL to LDL receptors, 26 the LDL receptor - related protein, 8 and proteoglycan 11, 27 and inhibits VLDL uptake by the liver, 28 antagonizing the accelerating effect of apoE on particle clearance.	bind
35265	8	8520	7	NULL	NULL	0	NULL	ApoC-III 	NULL		inhibits	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_146	11557678	6 ApoC-III reduces the binding of apoE-rich VLDL to LDL receptors, 26 the LDL receptor - related protein, 8 and proteoglycan 11, 27 and inhibits VLDL uptake by the liver, 28 antagonizing the accelerating effect of apoE on particle clearance.	bind
35266	9	8520	7	NULL	NULL	0	NULL	apoE	NULL		accelerates	NULL				particle clearance	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_146	11557678	6 ApoC-III reduces the binding of apoE-rich VLDL to LDL receptors, 26 the LDL receptor - related protein, 8 and proteoglycan 11, 27 and inhibits VLDL uptake by the liver, 28 antagonizing the accelerating effect of apoE on particle clearance.	bind
35267	10	8520	7	NULL	NULL	0	NULL	ApoC-III 	NULL		antagonize	NULL				statement 9	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_9_1494_s_146	11557678	6 ApoC-III reduces the binding of apoE-rich VLDL to LDL receptors, 26 the LDL receptor - related protein, 8 and proteoglycan 11, 27 and inhibits VLDL uptake by the liver, 28 antagonizing the accelerating effect of apoE on particle clearance.	bind
33655	1	8521	5	13	NULL	NULL	NULL	E1A	GP		bind					CBP/p300	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_48_31629_s_127	9822619	6 Because E1A binding to CBP/p300 is well characterized as a major mechanism by which adenovirus controls host cell function, it is likely that CBP/p300 is also a critical factor in the transcriptional response of PEPCK to hormones (see Fig.  2).	bind
35268	1	8521	7	NULL	NULL	0	NULL	E1A 	NULL		bind	NULL				CBP/p300	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_48_31629_s_127	9822619	6 Because E1A binding to CBP/p300 is well characterized as a major mechanism by which adenovirus controls host cell function, it is likely that CBP/p300 is also a critical factor in the transcriptional response of PEPCK to hormones (see Fig.  2).	bind
33658	1	8522	5	13	NULL	NULL	NULL	HSP90	GP		bind					eNOS	GP				NULL	cardiac myocytes	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1628_s_42	15231513	6 Estrogen, as well as hypoxia, stimulates HSP90 binding to eNOS in cardiac myocytes and vascular endothelial cells, 9 with subsequent regulation of NO release, PI3-Akt activation, and calcium sensitivity.	bind
33659	2	8522	5	13	NULL	NULL	NULL	HSP90	GP		bind					eNOS	GP				NULL	vascular endothelial cells	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1628_s_42	15231513	6 Estrogen, as well as hypoxia, stimulates HSP90 binding to eNOS in cardiac myocytes and vascular endothelial cells, 9 with subsequent regulation of NO release, PI3-Akt activation, and calcium sensitivity.	bind
33660	3	8522	5	13	NULL	NULL	NULL	estrogen	Chemical		stimulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1628_s_42	15231513	6 Estrogen, as well as hypoxia, stimulates HSP90 binding to eNOS in cardiac myocytes and vascular endothelial cells, 9 with subsequent regulation of NO release, PI3-Akt activation, and calcium sensitivity.	bind
33661	4	8522	5	13	NULL	NULL	NULL	estrogen	Chemical		stimulates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1628_s_42	15231513	6 Estrogen, as well as hypoxia, stimulates HSP90 binding to eNOS in cardiac myocytes and vascular endothelial cells, 9 with subsequent regulation of NO release, PI3-Akt activation, and calcium sensitivity.	bind
33662	5	8522	5	13	NULL	NULL	NULL	hypoxia	MedicalFinding		stimulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1628_s_42	15231513	6 Estrogen, as well as hypoxia, stimulates HSP90 binding to eNOS in cardiac myocytes and vascular endothelial cells, 9 with subsequent regulation of NO release, PI3-Akt activation, and calcium sensitivity.	bind
33663	6	8522	5	13	NULL	NULL	NULL	hypoxia	MedicalFinding		stimulates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1628_s_42	15231513	6 Estrogen, as well as hypoxia, stimulates HSP90 binding to eNOS in cardiac myocytes and vascular endothelial cells, 9 with subsequent regulation of NO release, PI3-Akt activation, and calcium sensitivity.	bind
33664	7	8522	5	13	NULL	NULL	NULL	estrogen	Chemical		regulates					NO	Chemical	release of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1628_s_42	15231513	6 Estrogen, as well as hypoxia, stimulates HSP90 binding to eNOS in cardiac myocytes and vascular endothelial cells, 9 with subsequent regulation of NO release, PI3-Akt activation, and calcium sensitivity.	bind
33665	8	8522	5	13	NULL	NULL	NULL	hypoxia	MedicalFinding		regulates					NO	Chemical	release of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1628_s_42	15231513	6 Estrogen, as well as hypoxia, stimulates HSP90 binding to eNOS in cardiac myocytes and vascular endothelial cells, 9 with subsequent regulation of NO release, PI3-Akt activation, and calcium sensitivity.	bind
33666	9	8522	5	13	NULL	NULL	NULL	estrogen	Chemical		regulates					PI3-Akt	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1628_s_42	15231513	6 Estrogen, as well as hypoxia, stimulates HSP90 binding to eNOS in cardiac myocytes and vascular endothelial cells, 9 with subsequent regulation of NO release, PI3-Akt activation, and calcium sensitivity.	bind
33667	10	8522	5	13	NULL	NULL	NULL	hypoxia	MedicalFinding		regulates					PI3-Akt	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1628_s_42	15231513	6 Estrogen, as well as hypoxia, stimulates HSP90 binding to eNOS in cardiac myocytes and vascular endothelial cells, 9 with subsequent regulation of NO release, PI3-Akt activation, and calcium sensitivity.	bind
33668	11	8522	5	13	NULL	NULL	NULL	estrogen	Chemical		regulates					calcium sensitivity	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1628_s_42	15231513	6 Estrogen, as well as hypoxia, stimulates HSP90 binding to eNOS in cardiac myocytes and vascular endothelial cells, 9 with subsequent regulation of NO release, PI3-Akt activation, and calcium sensitivity.	bind
33669	12	8522	5	13	NULL	NULL	NULL	hypoxia	MedicalFinding		regulates					calcium sensitivity	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1628_s_42	15231513	6 Estrogen, as well as hypoxia, stimulates HSP90 binding to eNOS in cardiac myocytes and vascular endothelial cells, 9 with subsequent regulation of NO release, PI3-Akt activation, and calcium sensitivity.	bind
35279	1	8522	7	NULL	NULL	0	NULL	HSP90	NULL		bind	NULL				eNOS	NULL				NULL	cardiac myocytes	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1628_s_42	15231513	6 Estrogen, as well as hypoxia, stimulates HSP90 binding to eNOS in cardiac myocytes and vascular endothelial cells, 9 with subsequent regulation of NO release, PI3-Akt activation, and calcium sensitivity.	bind
35283	2	8522	7	NULL	NULL	0	NULL	HSP90	NULL		bind	NULL				eNOS	NULL				NULL	vascular endothelial cells	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1628_s_42	15231513	6 Estrogen, as well as hypoxia, stimulates HSP90 binding to eNOS in cardiac myocytes and vascular endothelial cells, 9 with subsequent regulation of NO release, PI3-Akt activation, and calcium sensitivity.	bind
35284	3	8522	7	NULL	NULL	0	NULL	estrogen	NULL		stimulates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1628_s_42	15231513	6 Estrogen, as well as hypoxia, stimulates HSP90 binding to eNOS in cardiac myocytes and vascular endothelial cells, 9 with subsequent regulation of NO release, PI3-Akt activation, and calcium sensitivity.	bind
35285	4	8522	7	NULL	NULL	0	NULL	estrogen	NULL		stimulates	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1628_s_42	15231513	6 Estrogen, as well as hypoxia, stimulates HSP90 binding to eNOS in cardiac myocytes and vascular endothelial cells, 9 with subsequent regulation of NO release, PI3-Akt activation, and calcium sensitivity.	bind
35286	5	8522	7	NULL	NULL	0	NULL	hypoxia	NULL		stimulates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1628_s_42	15231513	6 Estrogen, as well as hypoxia, stimulates HSP90 binding to eNOS in cardiac myocytes and vascular endothelial cells, 9 with subsequent regulation of NO release, PI3-Akt activation, and calcium sensitivity.	bind
35287	6	8522	7	NULL	NULL	0	NULL	hypoxia	NULL		stimulates	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1628_s_42	15231513	6 Estrogen, as well as hypoxia, stimulates HSP90 binding to eNOS in cardiac myocytes and vascular endothelial cells, 9 with subsequent regulation of NO release, PI3-Akt activation, and calcium sensitivity.	bind
35288	7	8522	7	10	NULL	0	NULL	estrogen			regulates					NO 		release of 			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1628_s_42	15231513	6 Estrogen, as well as hypoxia, stimulates HSP90 binding to eNOS in cardiac myocytes and vascular endothelial cells, 9 with subsequent regulation of NO release, PI3-Akt activation, and calcium sensitivity.	bind
35289	8	8522	7	10	NULL	0	NULL	hypoxia			regulates					NO 		release of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1628_s_42	15231513	6 Estrogen, as well as hypoxia, stimulates HSP90 binding to eNOS in cardiac myocytes and vascular endothelial cells, 9 with subsequent regulation of NO release, PI3-Akt activation, and calcium sensitivity.	bind
35290	9	8522	7	NULL	NULL	0	NULL	estrogen	NULL		activates	NULL				PI3-Akt	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1628_s_42	15231513	6 Estrogen, as well as hypoxia, stimulates HSP90 binding to eNOS in cardiac myocytes and vascular endothelial cells, 9 with subsequent regulation of NO release, PI3-Akt activation, and calcium sensitivity.	bind
35291	10	8522	7	NULL	NULL	0	NULL	hypoxia	NULL		activates	NULL				PI3-Akt	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1628_s_42	15231513	6 Estrogen, as well as hypoxia, stimulates HSP90 binding to eNOS in cardiac myocytes and vascular endothelial cells, 9 with subsequent regulation of NO release, PI3-Akt activation, and calcium sensitivity.	bind
35292	11	8522	7	NULL	NULL	0	NULL	estrogen	NULL		effect	NULL				calcium sensitivity	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1628_s_42	15231513	6 Estrogen, as well as hypoxia, stimulates HSP90 binding to eNOS in cardiac myocytes and vascular endothelial cells, 9 with subsequent regulation of NO release, PI3-Akt activation, and calcium sensitivity.	bind
35293	12	8522	7	NULL	NULL	0	NULL	hypoxia	NULL		effect	NULL				calcium sensitivity	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1628_s_42	15231513	6 Estrogen, as well as hypoxia, stimulates HSP90 binding to eNOS in cardiac myocytes and vascular endothelial cells, 9 with subsequent regulation of NO release, PI3-Akt activation, and calcium sensitivity.	bind
33670	1	8523	5	13	NULL	NULL	NULL	FGFRs	GP		bind					FGFs	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_5_1465_s_20	10329600	6 FGFRs bind to fibroblast growth factors (FGFs), which are known to regulate proliferation, survival, differentiation, and migration of a wide variety of cells.	bind
33671	2	8523	5	13	NULL	NULL	NULL	FGFs	GP		is					fibroblast growth factors	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_5_1465_s_20	10329600	6 FGFRs bind to fibroblast growth factors (FGFs), which are known to regulate proliferation, survival, differentiation, and migration of a wide variety of cells.	bind
33672	3	8523	5	13	NULL	NULL	NULL	FGFs	GP		regulates					cell proliferation	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_5_1465_s_20	10329600	6 FGFRs bind to fibroblast growth factors (FGFs), which are known to regulate proliferation, survival, differentiation, and migration of a wide variety of cells.	bind
33673	4	8523	5	13	NULL	NULL	NULL	FGFs	GP		regulates					cell survival	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_5_1465_s_20	10329600	6 FGFRs bind to fibroblast growth factors (FGFs), which are known to regulate proliferation, survival, differentiation, and migration of a wide variety of cells.	bind
33674	5	8523	5	13	NULL	NULL	NULL	FGFs	GP		regulates					cell differentiation	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_5_1465_s_20	10329600	6 FGFRs bind to fibroblast growth factors (FGFs), which are known to regulate proliferation, survival, differentiation, and migration of a wide variety of cells.	bind
33675	6	8523	5	13	NULL	NULL	NULL	FGFs	GP		regulates					cell migration	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_5_1465_s_20	10329600	6 FGFRs bind to fibroblast growth factors (FGFs), which are known to regulate proliferation, survival, differentiation, and migration of a wide variety of cells.	bind
35294	1	8523	7	NULL	NULL	0	NULL	FGFRs	NULL		bind to	NULL				FGFs	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_5_1465_s_20	10329600	6 FGFRs bind to fibroblast growth factors (FGFs), which are known to regulate proliferation, survival, differentiation, and migration of a wide variety of cells.	bind
35295	2	8523	7	10	NULL	0	NULL	FGFs			regulate					cell proliferation					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_5_1465_s_20	10329600	6 FGFRs bind to fibroblast growth factors (FGFs), which are known to regulate proliferation, survival, differentiation, and migration of a wide variety of cells.	bind
35296	3	8523	7	10	NULL	0	NULL	FGFs			regulate					cell survival					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_5_1465_s_20	10329600	6 FGFRs bind to fibroblast growth factors (FGFs), which are known to regulate proliferation, survival, differentiation, and migration of a wide variety of cells.	bind
35297	4	8523	7	NULL	NULL	0	NULL	FGFs	NULL		regulate	NULL				cell differentiation	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_5_1465_s_20	10329600	6 FGFRs bind to fibroblast growth factors (FGFs), which are known to regulate proliferation, survival, differentiation, and migration of a wide variety of cells.	bind
35298	5	8523	7	NULL	NULL	0	NULL	FGFs	NULL		regulate	NULL				cell migration	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_5_1465_s_20	10329600	6 FGFRs bind to fibroblast growth factors (FGFs), which are known to regulate proliferation, survival, differentiation, and migration of a wide variety of cells.	bind
35299	6	8523	7	NULL	NULL	0	NULL	FGFs	NULL		is	NULL				fibroblast growth factors	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_5_1465_s_20	10329600	6 FGFRs bind to fibroblast growth factors (FGFs), which are known to regulate proliferation, survival, differentiation, and migration of a wide variety of cells.	bind
33676	1	8524	5	13	NULL	NULL	NULL	nuclear protein	GP		bind					TH	GP			CRE	NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_70_2_219_s_176	10407170	6 in PC12 cells results in a decrease in the nuclear protein binding to the TH CRE.	bind
35300	1	8524	7	10	NULL	0	NULL	nuclear protein			bind					TH				CRE	NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_70_2_219_s_176	10407170	6 in PC12 cells results in a decrease in the nuclear protein binding to the TH CRE.	bind
33677	1	8525	5	13	NULL	NULL	NULL	protein C	GP		bind					phospholipid vesicles	CellComponent				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_275_8_10681521_s_8	10681521	6 mM MgCl(2),  sEPCR inhibited the binding of protein C and APC to phospholipid vesicles  (K(i) = 40 +/- 7 and 33 +/- 4 nM, respectively).	bind
33678	2	8525	5	13	NULL	NULL	NULL	APC	GP		bind					phospholipid vesicles	CellComponent				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_275_8_10681521_s_8	10681521	6 mM MgCl(2),  sEPCR inhibited the binding of protein C and APC to phospholipid vesicles  (K(i) = 40 +/- 7 and 33 +/- 4 nM, respectively).	bind
33679	3	8525	5	13	NULL	NULL	NULL	sEPCR	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_275_8_10681521_s_8	10681521	6 mM MgCl(2),  sEPCR inhibited the binding of protein C and APC to phospholipid vesicles  (K(i) = 40 +/- 7 and 33 +/- 4 nM, respectively).	bind
33680	4	8525	5	13	NULL	NULL	NULL	sEPCR	GP		inhibits					statement 2	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_275_8_10681521_s_8	10681521	6 mM MgCl(2),  sEPCR inhibited the binding of protein C and APC to phospholipid vesicles  (K(i) = 40 +/- 7 and 33 +/- 4 nM, respectively).	bind
35302	1	8525	7	NULL	NULL	0	NULL	protein C	NULL		bind	NULL				 phospholipid vesicles	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_275_8_10681521_s_8	10681521	6 mM MgCl(2),  sEPCR inhibited the binding of protein C and APC to phospholipid vesicles  (K(i) = 40 +/- 7 and 33 +/- 4 nM, respectively).	bind
35303	2	8525	7	NULL	NULL	0	NULL	APC	NULL		bind	NULL				phospholipid vesicles	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_275_8_10681521_s_8	10681521	6 mM MgCl(2),  sEPCR inhibited the binding of protein C and APC to phospholipid vesicles  (K(i) = 40 +/- 7 and 33 +/- 4 nM, respectively).	bind
35304	3	8525	7	NULL	NULL	0	NULL	sEPCR	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_275_8_10681521_s_8	10681521	6 mM MgCl(2),  sEPCR inhibited the binding of protein C and APC to phospholipid vesicles  (K(i) = 40 +/- 7 and 33 +/- 4 nM, respectively).	bind
35305	4	8525	7	NULL	NULL	0	NULL	sEPCR	NULL		inhibits	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_275_8_10681521_s_8	10681521	6 mM MgCl(2),  sEPCR inhibited the binding of protein C and APC to phospholipid vesicles  (K(i) = 40 +/- 7 and 33 +/- 4 nM, respectively).	bind
33707	1	8526	5	13	NULL	NULL	NULL	Grb-IRbeta/Grb10	GP		interacts with					insulin-like growth factor-1 receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_5_2659_s_314	9006901	6 O'NeillP  et al. ( 47) demonstrated interactions of Grb-IRbeta/Grb10 with insulin-like growth factor-1 receptors, whereas we showed binding to activated PDGF and EGF receptors.	bind
33708	2	8526	5	13	NULL	NULL	NULL	Grb-IRbeta/Grb10	GP		bind					PDGF receptor	GP	activated			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_5_2659_s_314	9006901	6 O'NeillP  et al. ( 47) demonstrated interactions of Grb-IRbeta/Grb10 with insulin-like growth factor-1 receptors, whereas we showed binding to activated PDGF and EGF receptors.	bind
33709	3	8526	5	13	NULL	NULL	NULL	Grb-IRbeta/Grb10	GP		bind					EGF receptor	GP	activated			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_5_2659_s_314	9006901	6 O'NeillP  et al. ( 47) demonstrated interactions of Grb-IRbeta/Grb10 with insulin-like growth factor-1 receptors, whereas we showed binding to activated PDGF and EGF receptors.	bind
35306	1	8526	7	NULL	NULL	0	NULL	Grb-IRbeta/Grb10	NULL		interacts with	NULL				insulin-like growth factor-1 receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_5_2659_s_314	9006901	6 O'NeillP  et al. ( 47) demonstrated interactions of Grb-IRbeta/Grb10 with insulin-like growth factor-1 receptors, whereas we showed binding to activated PDGF and EGF receptors.	bind
35307	2	8526	7	NULL	NULL	0	NULL	Grb-IRbeta/Grb10	NULL		bind	NULL				PDGF	NULL	activated			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_5_2659_s_314	9006901	6 O'NeillP  et al. ( 47) demonstrated interactions of Grb-IRbeta/Grb10 with insulin-like growth factor-1 receptors, whereas we showed binding to activated PDGF and EGF receptors.	bind
35308	3	8526	7	NULL	NULL	0	NULL	Grb-IRbeta/Grb10	NULL		bind	NULL				EGF receptors	NULL	activated			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_5_2659_s_314	9006901	6 O'NeillP  et al. ( 47) demonstrated interactions of Grb-IRbeta/Grb10 with insulin-like growth factor-1 receptors, whereas we showed binding to activated PDGF and EGF receptors.	bind
33710	1	8528	5	13	NULL	NULL	NULL				bind			StAR domain		cholesterol	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_7_682_s_25	16141411	6 The StAR domain binds cholesterol and stimulates its movement from donor vesicles to the acceptor membrane.	bind
33711	2	8528	5	13	NULL	NULL	NULL	cholesterol	Chemical		moves from					donor vesicles	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_7_682_s_25	16141411	6 The StAR domain binds cholesterol and stimulates its movement from donor vesicles to the acceptor membrane.	bind
33712	5	8528	5	13	NULL	NULL	NULL	statement 1	Process		stimulates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_7_682_s_25	16141411	6 The StAR domain binds cholesterol and stimulates its movement from donor vesicles to the acceptor membrane.	bind
33799	3	8528	5	13	NULL	NULL	NULL	cholesterol	Chemical		moves to					acceptor membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_7_682_s_25	16141411	6 The StAR domain binds cholesterol and stimulates its movement from donor vesicles to the acceptor membrane.	bind
33800	4	8528	5	13	NULL	NULL	NULL	statement 2	Process		occurs after					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_7_682_s_25	16141411	6 The StAR domain binds cholesterol and stimulates its movement from donor vesicles to the acceptor membrane.	bind
33801	6	8528	5	13	NULL	NULL	NULL	statement 1	Process		stimulates					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_7_682_s_25	16141411	6 The StAR domain binds cholesterol and stimulates its movement from donor vesicles to the acceptor membrane.	bind
35309	1	8528	7	NULL	NULL	0	NULL		NULL		binds	NULL		StAR domain		cholesterol	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_7_682_s_25	16141411	6 The StAR domain binds cholesterol and stimulates its movement from donor vesicles to the acceptor membrane.	bind
35310	2	8528	7	NULL	NULL	0	NULL	cholesterol	NULL		move from	NULL				donor vesicles	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_7_682_s_25	16141411	6 The StAR domain binds cholesterol and stimulates its movement from donor vesicles to the acceptor membrane.	bind
35311	3	8528	7	NULL	NULL	0	NULL	cholesterol	NULL		move to	NULL				acceptor membrane	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_7_682_s_25	16141411	6 The StAR domain binds cholesterol and stimulates its movement from donor vesicles to the acceptor membrane.	bind
35312	4	8528	7	NULL	NULL	0	NULL	statement 2	NULL		occurs after	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_7_682_s_25	16141411	6 The StAR domain binds cholesterol and stimulates its movement from donor vesicles to the acceptor membrane.	bind
35313	5	8528	7	NULL	NULL	0	NULL	statement 1	NULL		stimulates	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_7_682_s_25	16141411	6 The StAR domain binds cholesterol and stimulates its movement from donor vesicles to the acceptor membrane.	bind
33713	1	8529	5	13	NULL	NULL	NULL	ATP	Chemical		bind					F1	GP		epsilon subunit		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_48_40130_s_193	16203732	6 Therefore, we assume that ATP binding to the epsilon subunit may stabilize the folded-hairpin form of the epsilon subunit in F1 to shift the equilibrium from the extended form.	bind
33714	2	8529	5	13	NULL	NULL	NULL	statement 1	Process		stabilize		may			F1	GP	folded hairpin form of	epsilon subunit		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_48_40130_s_193	16203732	6 Therefore, we assume that ATP binding to the epsilon subunit may stabilize the folded-hairpin form of the epsilon subunit in F1 to shift the equilibrium from the extended form.	bind
35314	1	8529	7	NULL	NULL	0	NULL	ATP	NULL		bind	NULL				F1	NULL		epsilon subunit 		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_48_40130_s_193	16203732	6 Therefore, we assume that ATP binding to the epsilon subunit may stabilize the folded-hairpin form of the epsilon subunit in F1 to shift the equilibrium from the extended form.	bind
35315	2	8529	7	10	NULL	0	NULL	statement 1	NULL		stabilize	NULL	may			F1	NULL	folded-hairpin form of	epsilon subunit 		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_48_40130_s_193	16203732	6 Therefore, we assume that ATP binding to the epsilon subunit may stabilize the folded-hairpin form of the epsilon subunit in F1 to shift the equilibrium from the extended form.	bind
33716	1	8530	5	13	NULL	NULL	NULL	SATB1	GP		is required for					mature CD8-positive T lymphocytes	Cell	production of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_29_18440_s_338	9218488	6 These results suggest that SATB1 is required for production of mature CD8-positive T lymphocytes and are consistent with our suggestion that binding of SATB1 to the L2a element plays a role in regulating expression of the  CD8a gene.	bind
33717	2	8530	5	13	NULL	NULL	NULL	SATB1	GP		bind									L2a element	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_29_18440_s_338	9218488	6 These results suggest that SATB1 is required for production of mature CD8-positive T lymphocytes and are consistent with our suggestion that binding of SATB1 to the L2a element plays a role in regulating expression of the  CD8a gene.	bind
33718	3	8530	5	13	NULL	NULL	NULL	statement 2	Process		regulates					CD8a gene	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_29_18440_s_338	9218488	6 These results suggest that SATB1 is required for production of mature CD8-positive T lymphocytes and are consistent with our suggestion that binding of SATB1 to the L2a element plays a role in regulating expression of the  CD8a gene.	bind
35317	1	8530	7	NULL	NULL	0	NULL	SATB1	NULL		is required for	NULL				mature CD8-positive T lymphocytes 	NULL	production of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_29_18440_s_338	9218488	6 These results suggest that SATB1 is required for production of mature CD8-positive T lymphocytes and are consistent with our suggestion that binding of SATB1 to the L2a element plays a role in regulating expression of the  CD8a gene.	bind
35318	2	8530	7	NULL	NULL	0	NULL	SATB1	NULL		bind	NULL					NULL			L2a element	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_29_18440_s_338	9218488	6 These results suggest that SATB1 is required for production of mature CD8-positive T lymphocytes and are consistent with our suggestion that binding of SATB1 to the L2a element plays a role in regulating expression of the  CD8a gene.	bind
35319	3	8530	7	NULL	NULL	0	NULL	statement 2	NULL		regulates	NULL				CD8a gene	NULL	expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_29_18440_s_338	9218488	6 These results suggest that SATB1 is required for production of mature CD8-positive T lymphocytes and are consistent with our suggestion that binding of SATB1 to the L2a element plays a role in regulating expression of the  CD8a gene.	bind
33719	1	8531	5	13	NULL	NULL	NULL	Sp1	GP		induces					SMC genes	GP	repression of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_981_s_135	15486317	6 These results suggest that Sp1-induced repression of SMC genes may involve more complex mechanisms than simple binding of Sp1 to the G/C repressor and subsequent inhibition of cooperative interactions between CArG elements (see Discussion for a detailed consideration of this issue).	bind
33720	2	8531	5	13	NULL	NULL	NULL	Sp1	GP		bind					G/C repressor	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_981_s_135	15486317	6 These results suggest that Sp1-induced repression of SMC genes may involve more complex mechanisms than simple binding of Sp1 to the G/C repressor and subsequent inhibition of cooperative interactions between CArG elements (see Discussion for a detailed consideration of this issue).	bind
33721	3	8531	5	10	NULL	0	NULL				interacts with		cooperatively		CArG element					CArG element	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_981_s_135	15486317	6 These results suggest that Sp1-induced repression of SMC genes may involve more complex mechanisms than simple binding of Sp1 to the G/C repressor and subsequent inhibition of cooperative interactions between CArG elements (see Discussion for a detailed consideration of this issue).	bind
55801	4	8531	5	13	NULL	NULL	NULL	statement 1	Process		involve					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_981_s_135	15486317	6 These results suggest that Sp1-induced repression of SMC genes may involve more complex mechanisms than simple binding of Sp1 to the G/C repressor and subsequent inhibition of cooperative interactions between CArG elements (see Discussion for a detailed consideration of this issue).	bind
55802	5	8531	5	13	NULL	NULL	NULL	statement 1	Process		involve					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_981_s_135	15486317	6 These results suggest that Sp1-induced repression of SMC genes may involve more complex mechanisms than simple binding of Sp1 to the G/C repressor and subsequent inhibition of cooperative interactions between CArG elements (see Discussion for a detailed consideration of this issue).	bind
35320	1	8531	7	NULL	NULL	0	NULL	Sp1	NULL		induce	NULL				SMC genes	NULL	repression of			NULL		0	NULL	NULL	NULL	gw70_circulationres_95_10_981_s_135	15486317	6 These results suggest that Sp1-induced repression of SMC genes may involve more complex mechanisms than simple binding of Sp1 to the G/C repressor and subsequent inhibition of cooperative interactions between CArG elements (see Discussion for a detailed consideration of this issue).	bind
35321	2	8531	7	10	NULL	0	NULL	Sp1	NULL		bind	NULL				G/C repressor	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_981_s_135	15486317	6 These results suggest that Sp1-induced repression of SMC genes may involve more complex mechanisms than simple binding of Sp1 to the G/C repressor and subsequent inhibition of cooperative interactions between CArG elements (see Discussion for a detailed consideration of this issue).	bind
35322	3	8531	7	NULL	NULL	0	NULL		NULL		interacts	NULL	cooperatively		CArG elements		NULL			CArG elements	NULL		0	NULL	NULL	NULL	gw70_circulationres_95_10_981_s_135	15486317	6 These results suggest that Sp1-induced repression of SMC genes may involve more complex mechanisms than simple binding of Sp1 to the G/C repressor and subsequent inhibition of cooperative interactions between CArG elements (see Discussion for a detailed consideration of this issue).	bind
35323	4	8531	7	NULL	NULL	0	NULL	statement 1	NULL		involve	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_95_10_981_s_135	15486317	6 These results suggest that Sp1-induced repression of SMC genes may involve more complex mechanisms than simple binding of Sp1 to the G/C repressor and subsequent inhibition of cooperative interactions between CArG elements (see Discussion for a detailed consideration of this issue).	bind
35324	5	8531	7	NULL	NULL	0	NULL	statement 1	NULL		involve	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_95_10_981_s_135	15486317	6 These results suggest that Sp1-induced repression of SMC genes may involve more complex mechanisms than simple binding of Sp1 to the G/C repressor and subsequent inhibition of cooperative interactions between CArG elements (see Discussion for a detailed consideration of this issue).	bind
33722	1	8532	5	13	NULL	NULL	NULL	rA1	GP		bind					prothrombin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_31954_s_229	10924522	6) Based on a molecular model of the Al domain, conformationally constrained peptides were synthesized, which act synergistically to inhibit rA1 binding to prothrombin (Fig.  4,  A and  B) or PF2 binding to FXI (Fig.  6 ( A and  B), Table  I).	bind
33723	2	8532	5	13	NULL	NULL	NULL	PF2	GP		bind					FXI	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_31954_s_229	10924522	6) Based on a molecular model of the Al domain, conformationally constrained peptides were synthesized, which act synergistically to inhibit rA1 binding to prothrombin (Fig.  4,  A and  B) or PF2 binding to FXI (Fig.  6 ( A and  B), Table  I).	bind
33725	4	8532	5	13	NULL	NULL	NULL	peptides	GP	conformationally;; constrained	inhibits		synergistically			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_31954_s_229	10924522	6) Based on a molecular model of the Al domain, conformationally constrained peptides were synthesized, which act synergistically to inhibit rA1 binding to prothrombin (Fig.  4,  A and  B) or PF2 binding to FXI (Fig.  6 ( A and  B), Table  I).	bind
55803	3	8532	5	13	NULL	NULL	NULL	peptides	GP	conformationally constrained	inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_31954_s_229	10924522	6) Based on a molecular model of the Al domain, conformationally constrained peptides were synthesized, which act synergistically to inhibit rA1 binding to prothrombin (Fig.  4,  A and  B) or PF2 binding to FXI (Fig.  6 ( A and  B), Table  I).	bind
35325	1	8532	7	NULL	NULL	0	NULL	 rA1	NULL		bind	NULL				prothrombin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_41_31954_s_229	10924522	6) Based on a molecular model of the Al domain, conformationally constrained peptides were synthesized, which act synergistically to inhibit rA1 binding to prothrombin (Fig.  4,  A and  B) or PF2 binding to FXI (Fig.  6 ( A and  B), Table  I).	bind
35326	2	8532	7	NULL	NULL	0	NULL	PF2	NULL		bind	NULL				FXI	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_41_31954_s_229	10924522	6) Based on a molecular model of the Al domain, conformationally constrained peptides were synthesized, which act synergistically to inhibit rA1 binding to prothrombin (Fig.  4,  A and  B) or PF2 binding to FXI (Fig.  6 ( A and  B), Table  I).	bind
35327	3	8532	7	10	NULL	0	NULL	peptides		conformationally;; constrained	inhibit					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_31954_s_229	10924522	6) Based on a molecular model of the Al domain, conformationally constrained peptides were synthesized, which act synergistically to inhibit rA1 binding to prothrombin (Fig.  4,  A and  B) or PF2 binding to FXI (Fig.  6 ( A and  B), Table  I).	bind
35328	4	8532	7	10	NULL	0	NULL	peptides		conformationally;; constrained	inhibit					statement 2					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_31954_s_229	10924522	6) Based on a molecular model of the Al domain, conformationally constrained peptides were synthesized, which act synergistically to inhibit rA1 binding to prothrombin (Fig.  4,  A and  B) or PF2 binding to FXI (Fig.  6 ( A and  B), Table  I).	bind
34274	1	8533	5	13	NULL	NULL	NULL	p47 phox	GP		bind								target domains in cytosolic loop		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_316	11733522	6) Binding of p47 phox and p67 phox to their target domains in the cytosolic loop and at the root of the cytosolic tail is mediated by interactions other than those involving SH3 domains and proline-rich regions, the nature of which remains to be established.	bind
34275	2	8533	5	13	NULL	NULL	NULL	p67 phox	GP		bind								target domains in cytosolic loop		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_316	11733522	6) Binding of p47 phox and p67 phox to their target domains in the cytosolic loop and at the root of the cytosolic tail is mediated by interactions other than those involving SH3 domains and proline-rich regions, the nature of which remains to be established.	bind
34276	3	8533	5	13	NULL	NULL	NULL	p47 phox	GP		bind								root of the cytosolic tail		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_316	11733522	6) Binding of p47 phox and p67 phox to their target domains in the cytosolic loop and at the root of the cytosolic tail is mediated by interactions other than those involving SH3 domains and proline-rich regions, the nature of which remains to be established.	bind
34277	4	8533	5	13	NULL	NULL	NULL	p67 phox	GP		bind								root of the cytosolic tail		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_316	11733522	6) Binding of p47 phox and p67 phox to their target domains in the cytosolic loop and at the root of the cytosolic tail is mediated by interactions other than those involving SH3 domains and proline-rich regions, the nature of which remains to be established.	bind
34278	5	8533	5	13	NULL	NULL	NULL	statement 1	Process		is not mediated by								SH3 domains;;proline-rich regions		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_316	11733522	6) Binding of p47 phox and p67 phox to their target domains in the cytosolic loop and at the root of the cytosolic tail is mediated by interactions other than those involving SH3 domains and proline-rich regions, the nature of which remains to be established.	bind
34287	6	8533	5	13	NULL	NULL	NULL	statement 2	Process		is not mediated by								SH3 domains;;proline-rich regions		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_316	11733522	6) Binding of p47 phox and p67 phox to their target domains in the cytosolic loop and at the root of the cytosolic tail is mediated by interactions other than those involving SH3 domains and proline-rich regions, the nature of which remains to be established.	bind
34288	7	8533	5	13	NULL	NULL	NULL	statement 3	Process		is not mediated by								SH3 domains;;proline-rich regions		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_316	11733522	6) Binding of p47 phox and p67 phox to their target domains in the cytosolic loop and at the root of the cytosolic tail is mediated by interactions other than those involving SH3 domains and proline-rich regions, the nature of which remains to be established.	bind
34289	8	8533	5	13	NULL	NULL	NULL	statement 4	Process		is not mediated by								SH3 domains;;proline-rich regions		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_316	11733522	6) Binding of p47 phox and p67 phox to their target domains in the cytosolic loop and at the root of the cytosolic tail is mediated by interactions other than those involving SH3 domains and proline-rich regions, the nature of which remains to be established.	bind
35329	1	8533	7	NULL	NULL	0	NULL	p47	NULL		bind	NULL					NULL		domains in the cytosolic loop		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_316	11733522	6) Binding of p47 phox and p67 phox to their target domains in the cytosolic loop and at the root of the cytosolic tail is mediated by interactions other than those involving SH3 domains and proline-rich regions, the nature of which remains to be established.	bind
35330	2	8533	7	NULL	NULL	0	NULL	p67 phox 	NULL		bind	NULL					NULL		domains in the cytosolic loop		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_316	11733522	6) Binding of p47 phox and p67 phox to their target domains in the cytosolic loop and at the root of the cytosolic tail is mediated by interactions other than those involving SH3 domains and proline-rich regions, the nature of which remains to be established.	bind
35331	3	8533	7	NULL	NULL	0	NULL	p47 phox	NULL		bind	NULL					NULL		cytosolic tail		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_316	11733522	6) Binding of p47 phox and p67 phox to their target domains in the cytosolic loop and at the root of the cytosolic tail is mediated by interactions other than those involving SH3 domains and proline-rich regions, the nature of which remains to be established.	bind
35332	4	8533	7	NULL	NULL	0	NULL	p67 phox	NULL		bind	NULL					NULL		cytosolic tail		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_316	11733522	6) Binding of p47 phox and p67 phox to their target domains in the cytosolic loop and at the root of the cytosolic tail is mediated by interactions other than those involving SH3 domains and proline-rich regions, the nature of which remains to be established.	bind
35333	5	8533	7	NULL	NULL	0	NULL		NULL		does not mediate	NULL		SH3 domain		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_316	11733522	6) Binding of p47 phox and p67 phox to their target domains in the cytosolic loop and at the root of the cytosolic tail is mediated by interactions other than those involving SH3 domains and proline-rich regions, the nature of which remains to be established.	bind
35334	6	8533	7	NULL	NULL	0	NULL		NULL		does not mediate	NULL		SH3 domain		statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_316	11733522	6) Binding of p47 phox and p67 phox to their target domains in the cytosolic loop and at the root of the cytosolic tail is mediated by interactions other than those involving SH3 domains and proline-rich regions, the nature of which remains to be established.	bind
35335	7	8533	7	NULL	NULL	0	NULL		NULL		does not mediate	NULL		SH3 domain		statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_316	11733522	6) Binding of p47 phox and p67 phox to their target domains in the cytosolic loop and at the root of the cytosolic tail is mediated by interactions other than those involving SH3 domains and proline-rich regions, the nature of which remains to be established.	bind
35336	8	8533	7	NULL	NULL	0	NULL		NULL		does not mediate	NULL		SH3 domain		statement 4	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_316	11733522	6) Binding of p47 phox and p67 phox to their target domains in the cytosolic loop and at the root of the cytosolic tail is mediated by interactions other than those involving SH3 domains and proline-rich regions, the nature of which remains to be established.	bind
35337	9	8533	7	NULL	NULL	0	NULL		NULL		does not mediate	NULL		proline-rich region		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_316	11733522	6) Binding of p47 phox and p67 phox to their target domains in the cytosolic loop and at the root of the cytosolic tail is mediated by interactions other than those involving SH3 domains and proline-rich regions, the nature of which remains to be established.	bind
35338	10	8533	7	NULL	NULL	0	NULL		NULL		does not mediate	NULL		proline-rich region		statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_316	11733522	6) Binding of p47 phox and p67 phox to their target domains in the cytosolic loop and at the root of the cytosolic tail is mediated by interactions other than those involving SH3 domains and proline-rich regions, the nature of which remains to be established.	bind
35339	11	8533	7	NULL	NULL	0	NULL		NULL		does not mediate	NULL		proline-rich region		statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_316	11733522	6) Binding of p47 phox and p67 phox to their target domains in the cytosolic loop and at the root of the cytosolic tail is mediated by interactions other than those involving SH3 domains and proline-rich regions, the nature of which remains to be established.	bind
35340	12	8533	7	NULL	NULL	0	NULL		NULL		does not mediate	NULL		proline-rich region		statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_316	11733522	6) Binding of p47 phox and p67 phox to their target domains in the cytosolic loop and at the root of the cytosolic tail is mediated by interactions other than those involving SH3 domains and proline-rich regions, the nature of which remains to be established.	bind
33726	1	8534	5	13	NULL	NULL	NULL	GM1	Chemical		bind					Trk protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_40_26001_s_192	9748278	6) D-PDMP treatment causes down-regulation of endogenous gangliosides as well as binding of GM1 to the Trk protein.	bind
33727	2	8534	5	13	NULL	NULL	NULL	D-PDMP	Chemical		down regulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_40_26001_s_192	9748278	6) D-PDMP treatment causes down-regulation of endogenous gangliosides as well as binding of GM1 to the Trk protein.	bind
33728	3	8534	5	13	NULL	NULL	NULL	D-PDMP	Chemical		down regulates					gangliosides	Chemical	endogenous			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_40_26001_s_192	9748278	6) D-PDMP treatment causes down-regulation of endogenous gangliosides as well as binding of GM1 to the Trk protein.	bind
35341	1	8534	7	NULL	NULL	0	NULL	GM1	NULL		bind	NULL				Trk protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_40_26001_s_192	9748278	6) D-PDMP treatment causes down-regulation of endogenous gangliosides as well as binding of GM1 to the Trk protein.	bind
35342	2	8534	7	10	NULL	0	NULL	 D-PDMP			downregulates					gangliosides		endogenous			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_40_26001_s_192	9748278	6) D-PDMP treatment causes down-regulation of endogenous gangliosides as well as binding of GM1 to the Trk protein.	bind
35343	3	8534	7	10	NULL	0	NULL	D-PDMP			downregulates					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_40_26001_s_192	9748278	6) D-PDMP treatment causes down-regulation of endogenous gangliosides as well as binding of GM1 to the Trk protein.	bind
33729	1	8536	5	13	NULL	NULL	NULL	gammadelta T cells	Cell	proliferation of 	is induced by					CMV extracts	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_103_10_1437_s_217	10330426	6), CD1c (L161), and CD1d (51.1) did not block the proliferation of gammadelta T cells induced by CMV extracts (data not shown).	bind
33730	2	8536	5	13	NULL	NULL	NULL	CD1c	GP		does not block					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_103_10_1437_s_217	10330426	6), CD1c (L161), and CD1d (51.1) did not block the proliferation of gammadelta T cells induced by CMV extracts (data not shown).	bind
33731	3	8536	5	13	NULL	NULL	NULL	CD1d	GP		does not block					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_103_10_1437_s_217	10330426	6), CD1c (L161), and CD1d (51.1) did not block the proliferation of gammadelta T cells induced by CMV extracts (data not shown).	bind
35404	1	8536	7	NULL	NULL	0	NULL	CMV extracts	NULL		induce	NULL				gammadelta T cells	NULL	proliferation of			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_103_10_1437_s_217	10330426	6), CD1c (L161), and CD1d (51.1) did not block the proliferation of gammadelta T cells induced by CMV extracts (data not shown).	bind
35405	2	8536	7	10	NULL	0	NULL	CD1c			does not block					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_103_10_1437_s_217	10330426	6), CD1c (L161), and CD1d (51.1) did not block the proliferation of gammadelta T cells induced by CMV extracts (data not shown).	bind
35406	3	8536	7	NULL	NULL	0	NULL	CD1d	NULL		does not block	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_103_10_1437_s_217	10330426	6), CD1c (L161), and CD1d (51.1) did not block the proliferation of gammadelta T cells induced by CMV extracts (data not shown).	bind
33733	1	8537	5	13	NULL	NULL	NULL	trkA	GP		bind					NGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_5_1661_s_17	10550322	6, 7  The tyrosine kinase receptors selectively bind to their cognate ligands: trkA for nerve growth factor (NGF) and NT-3; trkB for BDNF, NT-4/5, and NT-3; and trkC for NT-3.	bind
33734	2	8537	5	13	NULL	NULL	NULL	NGF	GP		is					nerve growth factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_5_1661_s_17	10550322	6, 7  The tyrosine kinase receptors selectively bind to their cognate ligands: trkA for nerve growth factor (NGF) and NT-3; trkB for BDNF, NT-4/5, and NT-3; and trkC for NT-3.	bind
33735	3	8537	5	13	NULL	NULL	NULL	trkA	GP		bind					NT-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_5_1661_s_17	10550322	6, 7  The tyrosine kinase receptors selectively bind to their cognate ligands: trkA for nerve growth factor (NGF) and NT-3; trkB for BDNF, NT-4/5, and NT-3; and trkC for NT-3.	bind
33736	4	8537	5	13	NULL	NULL	NULL	trkB	GP		bind					BDNF	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_5_1661_s_17	10550322	6, 7  The tyrosine kinase receptors selectively bind to their cognate ligands: trkA for nerve growth factor (NGF) and NT-3; trkB for BDNF, NT-4/5, and NT-3; and trkC for NT-3.	bind
33737	5	8537	5	13	NULL	NULL	NULL	trkB	GP		bind					NT-4/5	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_5_1661_s_17	10550322	6, 7  The tyrosine kinase receptors selectively bind to their cognate ligands: trkA for nerve growth factor (NGF) and NT-3; trkB for BDNF, NT-4/5, and NT-3; and trkC for NT-3.	bind
33738	6	8537	5	13	NULL	NULL	NULL	trkB	GP		bind					NT-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_5_1661_s_17	10550322	6, 7  The tyrosine kinase receptors selectively bind to their cognate ligands: trkA for nerve growth factor (NGF) and NT-3; trkB for BDNF, NT-4/5, and NT-3; and trkC for NT-3.	bind
33739	7	8537	5	13	NULL	NULL	NULL	trkC	GP		bind					NT-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_5_1661_s_17	10550322	6, 7  The tyrosine kinase receptors selectively bind to their cognate ligands: trkA for nerve growth factor (NGF) and NT-3; trkB for BDNF, NT-4/5, and NT-3; and trkC for NT-3.	bind
35407	1	8537	7	NULL	NULL	0	NULL	 trkA	NULL		bind	NULL				NGF	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_5_1661_s_17	10550322	6, 7  The tyrosine kinase receptors selectively bind to their cognate ligands: trkA for nerve growth factor (NGF) and NT-3; trkB for BDNF, NT-4/5, and NT-3; and trkC for NT-3.	bind
35408	2	8537	7	NULL	NULL	0	NULL	trkA	NULL		bind	NULL				NT-3	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_5_1661_s_17	10550322	6, 7  The tyrosine kinase receptors selectively bind to their cognate ligands: trkA for nerve growth factor (NGF) and NT-3; trkB for BDNF, NT-4/5, and NT-3; and trkC for NT-3.	bind
35409	3	8537	7	NULL	NULL	0	NULL	trkB	NULL		bind	NULL				BDNF	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_5_1661_s_17	10550322	6, 7  The tyrosine kinase receptors selectively bind to their cognate ligands: trkA for nerve growth factor (NGF) and NT-3; trkB for BDNF, NT-4/5, and NT-3; and trkC for NT-3.	bind
35410	4	8537	7	NULL	NULL	0	NULL	trkB	NULL		bind	NULL				NT-4/5	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_5_1661_s_17	10550322	6, 7  The tyrosine kinase receptors selectively bind to their cognate ligands: trkA for nerve growth factor (NGF) and NT-3; trkB for BDNF, NT-4/5, and NT-3; and trkC for NT-3.	bind
35411	5	8537	7	NULL	NULL	0	NULL	trkB	NULL		bind	NULL				NT-3	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_5_1661_s_17	10550322	6, 7  The tyrosine kinase receptors selectively bind to their cognate ligands: trkA for nerve growth factor (NGF) and NT-3; trkB for BDNF, NT-4/5, and NT-3; and trkC for NT-3.	bind
35412	6	8537	7	NULL	NULL	0	NULL	trkC	NULL		bind	NULL				NT-3	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_5_1661_s_17	10550322	6, 7  The tyrosine kinase receptors selectively bind to their cognate ligands: trkA for nerve growth factor (NGF) and NT-3; trkB for BDNF, NT-4/5, and NT-3; and trkC for NT-3.	bind
35413	7	8537	7	NULL	NULL	0	NULL	NGF	NULL		is	NULL				nerve growth factor 	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_5_1661_s_17	10550322	6, 7  The tyrosine kinase receptors selectively bind to their cognate ligands: trkA for nerve growth factor (NGF) and NT-3; trkB for BDNF, NT-4/5, and NT-3; and trkC for NT-3.	bind
33740	1	8538	5	13	NULL	NULL	NULL	VEGF	GP		bind					type III tyrosine kinase receptors	GP				NULL	on vascular endothelial cells	NULL	NULL	NULL	NULL	gw60_amjpathol_156_1_159_s_12	10623663	6, 7  VEGF binds to two type III tyrosine kinase receptors on vascular endothelial cells, Flt-1 and KDR/Flk-1.	bind
33741	2	8538	5	13	NULL	NULL	NULL	VEGF	GP		bind					Flt-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_1_159_s_12	10623663	6, 7  VEGF binds to two type III tyrosine kinase receptors on vascular endothelial cells, Flt-1 and KDR/Flk-1.	bind
33742	3	8538	5	13	NULL	NULL	NULL	VEGF	GP		bind					KDR/Flk-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_1_159_s_12	10623663	6, 7  VEGF binds to two type III tyrosine kinase receptors on vascular endothelial cells, Flt-1 and KDR/Flk-1.	bind
35414	1	8538	7	NULL	NULL	0	NULL	VEGF	NULL		binds	NULL				type III tyrosine kinase receptors 	NULL				NULL	 vascular endothelial cells	0	NULL	NULL	NULL	gw60_amjpathol_156_1_159_s_12	10623663	6, 7  VEGF binds to two type III tyrosine kinase receptors on vascular endothelial cells, Flt-1 and KDR/Flk-1.	bind
35415	2	8538	7	NULL	NULL	0	NULL	VEGF	NULL		binds	NULL				Flt-1	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_1_159_s_12	10623663	6, 7  VEGF binds to two type III tyrosine kinase receptors on vascular endothelial cells, Flt-1 and KDR/Flk-1.	bind
35416	3	8538	7	NULL	NULL	0	NULL	VEGF	NULL		binds	NULL				KDR/Flk-1	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_1_159_s_12	10623663	6, 7  VEGF binds to two type III tyrosine kinase receptors on vascular endothelial cells, Flt-1 and KDR/Flk-1.	bind
33743	1	8539	5	13	NULL	NULL	NULL	LDL	GP		bind					versican	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_3_387_s_16	11884279	6, 7 The binding between LDL and versican or biglycan seems to be enhanced in the presence of lipoprotein lipase 8 or phospholipase A2.	bind
33744	2	8539	5	13	NULL	NULL	NULL	LDL	GP		bind					biglycan	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_3_387_s_16	11884279	6, 7 The binding between LDL and versican or biglycan seems to be enhanced in the presence of lipoprotein lipase 8 or phospholipase A2.	bind
33745	3	8539	5	13	NULL	NULL	NULL	statement 1	Process		is alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_3_387_s_16	11884279	6, 7 The binding between LDL and versican or biglycan seems to be enhanced in the presence of lipoprotein lipase 8 or phospholipase A2.	bind
33746	4	8539	5	13	NULL	NULL	NULL	lipoprotein lipase 8	GP		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_3_387_s_16	11884279	6, 7 The binding between LDL and versican or biglycan seems to be enhanced in the presence of lipoprotein lipase 8 or phospholipase A2.	bind
33747	5	8539	5	13	NULL	NULL	NULL	lipoprotein lipase 8	GP		enhances					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_3_387_s_16	11884279	6, 7 The binding between LDL and versican or biglycan seems to be enhanced in the presence of lipoprotein lipase 8 or phospholipase A2.	bind
33748	6	8539	5	13	NULL	NULL	NULL	phospholipase A2	GP		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_3_387_s_16	11884279	6, 7 The binding between LDL and versican or biglycan seems to be enhanced in the presence of lipoprotein lipase 8 or phospholipase A2.	bind
33749	7	8539	5	13	NULL	NULL	NULL	phospholipase A2	GP		enhances					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_3_387_s_16	11884279	6, 7 The binding between LDL and versican or biglycan seems to be enhanced in the presence of lipoprotein lipase 8 or phospholipase A2.	bind
35417	1	8539	7	NULL	NULL	0	NULL	LDL	NULL		bind	NULL				versican	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_3_387_s_16	11884279	6, 7 The binding between LDL and versican or biglycan seems to be enhanced in the presence of lipoprotein lipase 8 or phospholipase A2.	bind
35418	2	8539	7	NULL	NULL	0	NULL	LDL	NULL		bind	NULL				biglycan	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_3_387_s_16	11884279	6, 7 The binding between LDL and versican or biglycan seems to be enhanced in the presence of lipoprotein lipase 8 or phospholipase A2.	bind
35419	3	8539	7	NULL	NULL	0	NULL	lipoprotein lipase 8	NULL		enhance	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_3_387_s_16	11884279	6, 7 The binding between LDL and versican or biglycan seems to be enhanced in the presence of lipoprotein lipase 8 or phospholipase A2.	bind
35420	4	8539	7	NULL	NULL	0	NULL	lipoprotein lipase 8	NULL		enhance	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_3_387_s_16	11884279	6, 7 The binding between LDL and versican or biglycan seems to be enhanced in the presence of lipoprotein lipase 8 or phospholipase A2.	bind
35421	5	8539	7	NULL	NULL	0	NULL	phospholipase A2	NULL		enhance	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_3_387_s_16	11884279	6, 7 The binding between LDL and versican or biglycan seems to be enhanced in the presence of lipoprotein lipase 8 or phospholipase A2.	bind
35422	6	8539	7	NULL	NULL	0	NULL	phospholipase A2	NULL		enhance	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_3_387_s_16	11884279	6, 7 The binding between LDL and versican or biglycan seems to be enhanced in the presence of lipoprotein lipase 8 or phospholipase A2.	bind
33750	1	8540	5	13	NULL	NULL	NULL	PROb cells	Cell		bind					TGF-beta1	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1867_s_262	10362813	6, 8, 25, 31 Based on radioimmunoassay data, PROb cells bind TGF-beta1.	bind
35423	1	8540	7	NULL	NULL	0	NULL	PROb cells	NULL		bind	NULL				TGF-beta1	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_6_1867_s_262	10362813	6, 8, 25, 31 Based on radioimmunoassay data, PROb cells bind TGF-beta1.	bind
33917	1	8541	5	13	NULL	NULL	NULL	PDGF-BB	GP		induces					SMCs	Cell	phenotypic switching of vascular			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_132	15718508	6,11  B, PDGF-BB - induced phenotypic switching of vascular SMCs has been shown to be mediated  by multiple mechanisms, including activation of Elk-1, 45 KLF4-dependent downregulation of myocardin expression (Y. Liu and G.K. Owens, unpublished  data, 2004), and possible disruption of SRF binding to degenerate CArG elements.	bind
33926	2	8541	5	13	NULL	NULL	NULL	Elk-1	GP	activation of	mediates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_132	15718508	6,11  B, PDGF-BB - induced phenotypic switching of vascular SMCs has been shown to be mediated  by multiple mechanisms, including activation of Elk-1, 45 KLF4-dependent downregulation of myocardin expression (Y. Liu and G.K. Owens, unpublished  data, 2004), and possible disruption of SRF binding to degenerate CArG elements.	bind
33928	3	8541	5	13	NULL	NULL	NULL	myocardin	GP	downregulation of expression of	is dependent on					KLF4	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_132	15718508	6,11  B, PDGF-BB - induced phenotypic switching of vascular SMCs has been shown to be mediated  by multiple mechanisms, including activation of Elk-1, 45 KLF4-dependent downregulation of myocardin expression (Y. Liu and G.K. Owens, unpublished  data, 2004), and possible disruption of SRF binding to degenerate CArG elements.	bind
33929	4	8541	5	13	NULL	NULL	NULL	statement 3	Process		mediates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_132	15718508	6,11  B, PDGF-BB - induced phenotypic switching of vascular SMCs has been shown to be mediated  by multiple mechanisms, including activation of Elk-1, 45 KLF4-dependent downregulation of myocardin expression (Y. Liu and G.K. Owens, unpublished  data, 2004), and possible disruption of SRF binding to degenerate CArG elements.	bind
33931	5	8541	5	13	NULL	NULL	NULL	SRF	GP		bind							degenerate		CArG elements	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_132	15718508	6,11  B, PDGF-BB - induced phenotypic switching of vascular SMCs has been shown to be mediated  by multiple mechanisms, including activation of Elk-1, 45 KLF4-dependent downregulation of myocardin expression (Y. Liu and G.K. Owens, unpublished  data, 2004), and possible disruption of SRF binding to degenerate CArG elements.	bind
33933	6	8541	5	13	NULL	NULL	NULL	statement 5	Process	disruption of	mediates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_132	15718508	6,11  B, PDGF-BB - induced phenotypic switching of vascular SMCs has been shown to be mediated  by multiple mechanisms, including activation of Elk-1, 45 KLF4-dependent downregulation of myocardin expression (Y. Liu and G.K. Owens, unpublished  data, 2004), and possible disruption of SRF binding to degenerate CArG elements.	bind
35424	1	8541	7	NULL	NULL	0	NULL	PDGF-BB	NULL		induce	NULL				vascular SMCs 	NULL	phenotypic switching of			NULL		0	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_132	15718508	6,11  B, PDGF-BB - induced phenotypic switching of vascular SMCs has been shown to be mediated  by multiple mechanisms, including activation of Elk-1, 45 KLF4-dependent downregulation of myocardin expression (Y. Liu and G.K. Owens, unpublished  data, 2004), and possible disruption of SRF binding to degenerate CArG elements.	bind
35425	2	8541	7	NULL	NULL	0	NULL	Elk-1	NULL	activation of	mediates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_132	15718508	6,11  B, PDGF-BB - induced phenotypic switching of vascular SMCs has been shown to be mediated  by multiple mechanisms, including activation of Elk-1, 45 KLF4-dependent downregulation of myocardin expression (Y. Liu and G.K. Owens, unpublished  data, 2004), and possible disruption of SRF binding to degenerate CArG elements.	bind
35426	3	8541	7	NULL	NULL	0	NULL	 KLF4	NULL		downregulates	NULL				myocardin	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_132	15718508	6,11  B, PDGF-BB - induced phenotypic switching of vascular SMCs has been shown to be mediated  by multiple mechanisms, including activation of Elk-1, 45 KLF4-dependent downregulation of myocardin expression (Y. Liu and G.K. Owens, unpublished  data, 2004), and possible disruption of SRF binding to degenerate CArG elements.	bind
35427	4	8541	7	NULL	NULL	0	NULL	statement 3	NULL		mediates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_132	15718508	6,11  B, PDGF-BB - induced phenotypic switching of vascular SMCs has been shown to be mediated  by multiple mechanisms, including activation of Elk-1, 45 KLF4-dependent downregulation of myocardin expression (Y. Liu and G.K. Owens, unpublished  data, 2004), and possible disruption of SRF binding to degenerate CArG elements.	bind
35428	5	8541	7	NULL	NULL	0	NULL	SRF	NULL	binding of	degenerate	NULL					NULL			CArG elements	NULL		0	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_132	15718508	6,11  B, PDGF-BB - induced phenotypic switching of vascular SMCs has been shown to be mediated  by multiple mechanisms, including activation of Elk-1, 45 KLF4-dependent downregulation of myocardin expression (Y. Liu and G.K. Owens, unpublished  data, 2004), and possible disruption of SRF binding to degenerate CArG elements.	bind
35429	6	8541	7	NULL	NULL	0	NULL	statement 5	NULL	disruption of	mediates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_132	15718508	6,11  B, PDGF-BB - induced phenotypic switching of vascular SMCs has been shown to be mediated  by multiple mechanisms, including activation of Elk-1, 45 KLF4-dependent downregulation of myocardin expression (Y. Liu and G.K. Owens, unpublished  data, 2004), and possible disruption of SRF binding to degenerate CArG elements.	bind
33935	1	8542	5	13	NULL	NULL	NULL	VEGF	GP	mutant	bind			C156S		VEGFR-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_10_1098_s_26	12714562	6,13,16   In addition to the naturally occurring forms, Joukov et al 18 have generated a mutant factor (VEGF-C156S) that binds to VEGFR-3 but not to VEGFR-2.	bind
33936	2	8542	5	13	NULL	NULL	NULL	VEGF	GP	mutant	does not bind			C156S		VEGFR-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_10_1098_s_26	12714562	6,13,16   In addition to the naturally occurring forms, Joukov et al 18 have generated a mutant factor (VEGF-C156S) that binds to VEGFR-3 but not to VEGFR-2.	bind
35430	1	8542	7	NULL	NULL	0	NULL	VEGF	NULL		bind	NULL		C156S		 VEGFR-3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_92_10_1098_s_26	12714562	6,13,16   In addition to the naturally occurring forms, Joukov et al 18 have generated a mutant factor (VEGF-C156S) that binds to VEGFR-3 but not to VEGFR-2.	bind
35431	2	8542	7	NULL	NULL	0	NULL	VEGF	NULL		does not bind	NULL		C156S		VEGFR-2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_92_10_1098_s_26	12714562	6,13,16   In addition to the naturally occurring forms, Joukov et al 18 have generated a mutant factor (VEGF-C156S) that binds to VEGFR-3 but not to VEGFR-2.	bind
33938	1	8543	5	13	NULL	NULL	NULL	MCP-1	GP		bind					CCR2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_9_1177_s_183	16574901	6,7  The signaling events initiated by MCP-1 binding to CCR2 probably leads to transcriptional activation of genes for which products could lead to pathophysiological changes.	bind
33939	2	8543	5	13	NULL	NULL	NULL	statement 1	Process		initiates					signaling events	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_9_1177_s_183	16574901	6,7  The signaling events initiated by MCP-1 binding to CCR2 probably leads to transcriptional activation of genes for which products could lead to pathophysiological changes.	bind
33940	3	8543	5	13	NULL	NULL	NULL	statement 2	Process		leads to		probably			genes	GP	transcriptional activation of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_9_1177_s_183	16574901	6,7  The signaling events initiated by MCP-1 binding to CCR2 probably leads to transcriptional activation of genes for which products could lead to pathophysiological changes.	bind
35432	1	8543	7	NULL	NULL	0	NULL	MCP-1	NULL		bind	NULL				CCR2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_9_1177_s_183	16574901	6,7  The signaling events initiated by MCP-1 binding to CCR2 probably leads to transcriptional activation of genes for which products could lead to pathophysiological changes.	bind
35433	2	8543	7	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				genes	NULL	transcriptional activation of			NULL		0	NULL	NULL	NULL	gw70_circulationres_98_9_1177_s_183	16574901	6,7  The signaling events initiated by MCP-1 binding to CCR2 probably leads to transcriptional activation of genes for which products could lead to pathophysiological changes.	bind
35434	3	8543	7	NULL	NULL	0	NULL	statement 1	NULL		initiates	NULL				signaling events	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_9_1177_s_183	16574901	6,7  The signaling events initiated by MCP-1 binding to CCR2 probably leads to transcriptional activation of genes for which products could lead to pathophysiological changes.	bind
33947	1	8545	5	13	NULL	NULL	NULL	growth factors	GP		activates					Akt	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_2_431_s_13	11485901	6- 9 Activation of Akt by growth factors depends on the integrity of the PH domain, which binds to the PI 3-kinase product, PI(3,4,5)P3, and phosphorylation of Thr-308 and Ser-473 by PDK1 and PDK2/ILK, respectively.	bind
33948	2	8545	5	13	NULL	NULL	NULL	statement 1	Process		depends on					Akt	GP	 integrity of	PH domain		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_2_431_s_13	11485901	6- 9 Activation of Akt by growth factors depends on the integrity of the PH domain, which binds to the PI 3-kinase product, PI(3,4,5)P3, and phosphorylation of Thr-308 and Ser-473 by PDK1 and PDK2/ILK, respectively.	bind
33949	3	8545	5	13	NULL	NULL	NULL	Akt	GP		bind			PH domain		PI(3,4,5)P3	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_2_431_s_13	11485901	6- 9 Activation of Akt by growth factors depends on the integrity of the PH domain, which binds to the PI 3-kinase product, PI(3,4,5)P3, and phosphorylation of Thr-308 and Ser-473 by PDK1 and PDK2/ILK, respectively.	bind
33950	4	8545	5	13	NULL	NULL	NULL	PI(3,4,5)P3	Chemical		is a product of					PI 3-kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_2_431_s_13	11485901	6- 9 Activation of Akt by growth factors depends on the integrity of the PH domain, which binds to the PI 3-kinase product, PI(3,4,5)P3, and phosphorylation of Thr-308 and Ser-473 by PDK1 and PDK2/ILK, respectively.	bind
33951	5	8545	5	13	NULL	NULL	NULL	Akt	GP		is phosphorylated by			Thr-308		PDK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_2_431_s_13	11485901	6- 9 Activation of Akt by growth factors depends on the integrity of the PH domain, which binds to the PI 3-kinase product, PI(3,4,5)P3, and phosphorylation of Thr-308 and Ser-473 by PDK1 and PDK2/ILK, respectively.	bind
33952	6	8545	5	13	NULL	NULL	NULL	Akt	GP		is phosphorylated by			Ser-473		PDK2/ILK	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_2_431_s_13	11485901	6- 9 Activation of Akt by growth factors depends on the integrity of the PH domain, which binds to the PI 3-kinase product, PI(3,4,5)P3, and phosphorylation of Thr-308 and Ser-473 by PDK1 and PDK2/ILK, respectively.	bind
33953	7	8545	5	13	NULL	NULL	NULL	statement 1	Process		depends on					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_2_431_s_13	11485901	6- 9 Activation of Akt by growth factors depends on the integrity of the PH domain, which binds to the PI 3-kinase product, PI(3,4,5)P3, and phosphorylation of Thr-308 and Ser-473 by PDK1 and PDK2/ILK, respectively.	bind
33954	8	8545	5	13	NULL	NULL	NULL	statement 1	Process		depends on					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_2_431_s_13	11485901	6- 9 Activation of Akt by growth factors depends on the integrity of the PH domain, which binds to the PI 3-kinase product, PI(3,4,5)P3, and phosphorylation of Thr-308 and Ser-473 by PDK1 and PDK2/ILK, respectively.	bind
35436	1	8545	7	NULL	NULL	0	NULL	 growth factors	NULL		activates	NULL				Akt	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_2_431_s_13	11485901	6- 9 Activation of Akt by growth factors depends on the integrity of the PH domain, which binds to the PI 3-kinase product, PI(3,4,5)P3, and phosphorylation of Thr-308 and Ser-473 by PDK1 and PDK2/ILK, respectively.	bind
35439	2	8545	7	NULL	NULL	0	NULL	statement 1	NULL		depends on	NULL					NULL	integrity of	PH domain		NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_2_431_s_13	11485901	6- 9 Activation of Akt by growth factors depends on the integrity of the PH domain, which binds to the PI 3-kinase product, PI(3,4,5)P3, and phosphorylation of Thr-308 and Ser-473 by PDK1 and PDK2/ILK, respectively.	bind
35443	3	8545	7	NULL	NULL	0	NULL		NULL		binds to	NULL		PH domain		 PI 3-kinase	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_2_431_s_13	11485901	6- 9 Activation of Akt by growth factors depends on the integrity of the PH domain, which binds to the PI 3-kinase product, PI(3,4,5)P3, and phosphorylation of Thr-308 and Ser-473 by PDK1 and PDK2/ILK, respectively.	bind
35446	4	8545	7	NULL	NULL	0	NULL		NULL		binds to	NULL		PH domain		PI(3,4,5)P3	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_2_431_s_13	11485901	6- 9 Activation of Akt by growth factors depends on the integrity of the PH domain, which binds to the PI 3-kinase product, PI(3,4,5)P3, and phosphorylation of Thr-308 and Ser-473 by PDK1 and PDK2/ILK, respectively.	bind
35450	5	8545	7	NULL	NULL	0	NULL	PDK1	NULL		phosphorylates	NULL					NULL		Thr-308		NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_2_431_s_13	11485901	6- 9 Activation of Akt by growth factors depends on the integrity of the PH domain, which binds to the PI 3-kinase product, PI(3,4,5)P3, and phosphorylation of Thr-308 and Ser-473 by PDK1 and PDK2/ILK, respectively.	bind
35452	6	8545	7	NULL	NULL	0	NULL	PDK2/ILK	NULL		phosphorylates	NULL					NULL		Ser-473		NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_2_431_s_13	11485901	6- 9 Activation of Akt by growth factors depends on the integrity of the PH domain, which binds to the PI 3-kinase product, PI(3,4,5)P3, and phosphorylation of Thr-308 and Ser-473 by PDK1 and PDK2/ILK, respectively.	bind
35562	7	8545	7	NULL	NULL	0	NULL	statement 1	NULL		depends on	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_2_431_s_13	11485901	6- 9 Activation of Akt by growth factors depends on the integrity of the PH domain, which binds to the PI 3-kinase product, PI(3,4,5)P3, and phosphorylation of Thr-308 and Ser-473 by PDK1 and PDK2/ILK, respectively.	bind
35563	8	8545	7	NULL	NULL	0	NULL	statement 1	NULL		depends on	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_2_431_s_13	11485901	6- 9 Activation of Akt by growth factors depends on the integrity of the PH domain, which binds to the PI 3-kinase product, PI(3,4,5)P3, and phosphorylation of Thr-308 and Ser-473 by PDK1 and PDK2/ILK, respectively.	bind
33955	1	8546	5	13	NULL	NULL	NULL	6- 9alpha-DG	GP		linked to		noncovalently			beta-DG	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_5_1749_s_16	10793086	6- 9alpha-DG remains noncovalently linked to beta-DG, which through its cytoplasmic tail, binds directly to the C-terminal portion of dystrophin 10, 11  whereas the N-terminal domain of dystrophin binds to the subsarcolemmal actin cytoskeleton.	bind
33956	2	8546	5	13	NULL	NULL	NULL	beta-DG	GP		bind		directly	cytoplasmic tail		dystrophin	GP		C-terminal portion		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_5_1749_s_16	10793086	6- 9alpha-DG remains noncovalently linked to beta-DG, which through its cytoplasmic tail, binds directly to the C-terminal portion of dystrophin 10, 11  whereas the N-terminal domain of dystrophin binds to the subsarcolemmal actin cytoskeleton.	bind
33957	3	8546	5	13	NULL	NULL	NULL	dystrophin	GP		bind			N-terminal domain		subsarcolemmal actin cytoskeleton	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_5_1749_s_16	10793086	6- 9alpha-DG remains noncovalently linked to beta-DG, which through its cytoplasmic tail, binds directly to the C-terminal portion of dystrophin 10, 11  whereas the N-terminal domain of dystrophin binds to the subsarcolemmal actin cytoskeleton.	bind
35460	1	8546	7	NULL	NULL	0	NULL	9alpha-DG	NULL		linked to	NULL	noncovalently			beta-DG	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_5_1749_s_16	10793086	6- 9alpha-DG remains noncovalently linked to beta-DG, which through its cytoplasmic tail, binds directly to the C-terminal portion of dystrophin 10, 11  whereas the N-terminal domain of dystrophin binds to the subsarcolemmal actin cytoskeleton.	bind
35462	2	8546	7	NULL	NULL	0	NULL	beta-DG	NULL		binds	NULL	directly	cytoplasmic tail		dystrophin	NULL		C-terminal		NULL		0	NULL	NULL	NULL	gw60_amjpathol_156_5_1749_s_16	10793086	6- 9alpha-DG remains noncovalently linked to beta-DG, which through its cytoplasmic tail, binds directly to the C-terminal portion of dystrophin 10, 11  whereas the N-terminal domain of dystrophin binds to the subsarcolemmal actin cytoskeleton.	bind
35463	3	8546	7	10	NULL	0	NULL	dystrophin	NULL		binds to	NULL		N-terminal domain 		actin cytoskeleton	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_156_5_1749_s_16	10793086	6- 9alpha-DG remains noncovalently linked to beta-DG, which through its cytoplasmic tail, binds directly to the C-terminal portion of dystrophin 10, 11  whereas the N-terminal domain of dystrophin binds to the subsarcolemmal actin cytoskeleton.	bind
33958	1	8547	5	13	NULL	NULL	NULL	L-selectin	GP		bind		high affinity			HEV-associated ligands	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40226_s_18	10956661	6- O-Sulfation on galactose and  N-acetylglucosamine ( i.e. GlcNAc-6-SO4 and Gal-6-SO4) which is found in the context of sialyl Lewis X, is necessary for high affinity binding between L-selectin and these HEV-associated ligands ( 9).	bind
33959	2	8547	5	13	NULL	NULL	NULL	GlcNAc-6-SO4	Chemical		is					6- O-Sulfation on N-acetylglucosamine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40226_s_18	10956661	6- O-Sulfation on galactose and  N-acetylglucosamine ( i.e. GlcNAc-6-SO4 and Gal-6-SO4) which is found in the context of sialyl Lewis X, is necessary for high affinity binding between L-selectin and these HEV-associated ligands ( 9).	bind
33960	3	8547	5	13	NULL	NULL	NULL	Gal-6-SO4	Chemical		is					6- O-Sulfation on galactose	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40226_s_18	10956661	6- O-Sulfation on galactose and  N-acetylglucosamine ( i.e. GlcNAc-6-SO4 and Gal-6-SO4) which is found in the context of sialyl Lewis X, is necessary for high affinity binding between L-selectin and these HEV-associated ligands ( 9).	bind
35465	1	8547	7	NULL	NULL	0	NULL	L-selectin	NULL		bind	NULL	high affinity			HEV-associated ligands	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40226_s_18	10956661	6- O-Sulfation on galactose and  N-acetylglucosamine ( i.e. GlcNAc-6-SO4 and Gal-6-SO4) which is found in the context of sialyl Lewis X, is necessary for high affinity binding between L-selectin and these HEV-associated ligands ( 9).	bind
35467	2	8547	7	10	NULL	0	NULL	GlcNAc-6-SO4			is 					6- O-Sulfation on N-acetylglucosamine					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40226_s_18	10956661	6- O-Sulfation on galactose and  N-acetylglucosamine ( i.e. GlcNAc-6-SO4 and Gal-6-SO4) which is found in the context of sialyl Lewis X, is necessary for high affinity binding between L-selectin and these HEV-associated ligands ( 9).	bind
35468	3	8547	7	10	NULL	0	NULL	Gal-6-SO4			is					6- O-Sulfation on galactose					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40226_s_18	10956661	6- O-Sulfation on galactose and  N-acetylglucosamine ( i.e. GlcNAc-6-SO4 and Gal-6-SO4) which is found in the context of sialyl Lewis X, is necessary for high affinity binding between L-selectin and these HEV-associated ligands ( 9).	bind
33965	1	8549	5	13	NULL	NULL	NULL	Ins(1,4,5)P3	Chemical		bind					receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_4_1262_s_174	15249226	6-Deoxy-Ins(1,3,4,5)P4, however, inhibits the binding of [3]Ins(1,4,5)P3 to its receptor only slightly less effectively than Ins(1,3,4,5)P4.	bind
33966	2	8549	5	13	NULL	NULL	NULL	6-Deoxy-Ins(1,3,4,5)P4	Chemical		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_4_1262_s_174	15249226	6-Deoxy-Ins(1,3,4,5)P4, however, inhibits the binding of [3]Ins(1,4,5)P3 to its receptor only slightly less effectively than Ins(1,3,4,5)P4.	bind
33967	3	8549	5	13	NULL	NULL	NULL	Ins(1,3,4,5)P4	Chemical		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_4_1262_s_174	15249226	6-Deoxy-Ins(1,3,4,5)P4, however, inhibits the binding of [3]Ins(1,4,5)P3 to its receptor only slightly less effectively than Ins(1,3,4,5)P4.	bind
33968	4	8549	5	13	NULL	NULL	NULL	statement 2	Process		less effective than					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_4_1262_s_174	15249226	6-Deoxy-Ins(1,3,4,5)P4, however, inhibits the binding of [3]Ins(1,4,5)P3 to its receptor only slightly less effectively than Ins(1,3,4,5)P4.	bind
35470	1	8549	7	NULL	NULL	0	NULL	[3]Ins(1,4,5)P3	NULL		binds	NULL				 receptor	NULL				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_4_1262_s_174	15249226	6-Deoxy-Ins(1,3,4,5)P4, however, inhibits the binding of [3]Ins(1,4,5)P3 to its receptor only slightly less effectively than Ins(1,3,4,5)P4.	bind
35472	3	8549	7	NULL	NULL	0	NULL	6-Deoxy-Ins(1,3,4,5)P4	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_4_1262_s_174	15249226	6-Deoxy-Ins(1,3,4,5)P4, however, inhibits the binding of [3]Ins(1,4,5)P3 to its receptor only slightly less effectively than Ins(1,3,4,5)P4.	bind
35473	2	8549	7	NULL	NULL	0	NULL	Ins(1,3,4,5)P4	NULL		inhibits	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_4_1262_s_174	15249226	6-Deoxy-Ins(1,3,4,5)P4, however, inhibits the binding of [3]Ins(1,4,5)P3 to its receptor only slightly less effectively than Ins(1,3,4,5)P4.	bind
35474	5	8549	7	NULL	NULL	0	NULL	statement 3	NULL		is less effictive than	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_320_4_1262_s_174	15249226	6-Deoxy-Ins(1,3,4,5)P4, however, inhibits the binding of [3]Ins(1,4,5)P3 to its receptor only slightly less effectively than Ins(1,3,4,5)P4.	bind
33969	1	8550	5	13	NULL	NULL	NULL	6-Hydroxy-D-nicotine oxidase	GP		is a type of					monomeric protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_51_51307_s_24	14534317	6-Hydroxy-D-nicotine oxidase is a monomeric protein with FAD covalently bound to a histidine  residue.	bind
33970	2	8550	5	13	NULL	NULL	NULL	FAD	NucleicAcid		bind		covalently						histidine residue		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_51_51307_s_24	14534317	6-Hydroxy-D-nicotine oxidase is a monomeric protein with FAD covalently bound to a histidine  residue.	bind
33971	3	8550	5	13	NULL	NULL	NULL	6-Hydroxy-D-nicotine oxidase	GP		contains					statement 2	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_51_51307_s_24	14534317	6-Hydroxy-D-nicotine oxidase is a monomeric protein with FAD covalently bound to a histidine  residue.	bind
35475	1	8550	7	NULL	NULL	0	NULL	6-Hydroxy-D-nicotine oxidase	NULL		contains	NULL				FAD	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_51_51307_s_24	14534317	6-Hydroxy-D-nicotine oxidase is a monomeric protein with FAD covalently bound to a histidine  residue.	bind
35476	2	8550	7	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL	covalently				NULL		histidine residue		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_51_51307_s_24	14534317	6-Hydroxy-D-nicotine oxidase is a monomeric protein with FAD covalently bound to a histidine  residue.	bind
35477	3	8550	7	NULL	NULL	0	NULL	6-Hydroxy-D-nicotine oxidase	NULL		is a type of	NULL				monomeric protein	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_51_51307_s_24	14534317	6-Hydroxy-D-nicotine oxidase is a monomeric protein with FAD covalently bound to a histidine  residue.	bind
33972	1	8551	5	13	NULL	NULL	NULL	6-Mer heparin	Chemical		bind					GST-Tat	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_40_28198_s_8	10497173	6-Mer heparin binds GST-Tat with a dissociation constant ( K d) equal to 0.7  plus-or-minus  0.4 muM and a molar oligosaccharide:GST-Tat ratio of about 1:1.	bind
35478	1	8551	7	NULL	NULL	0	NULL	6-Mer heparin	NULL		binds	NULL				GST-Tat	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_40_28198_s_8	10497173	6-Mer heparin binds GST-Tat with a dissociation constant ( K d) equal to 0.7  plus-or-minus  0.4 muM and a molar oligosaccharide:GST-Tat ratio of about 1:1.	bind
33973	1	8553	5	13	NULL	NULL	NULL	FGF-2	GP		induces					FGFR-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24653_s_180	10816596	6-O-Desulfated Heparin Is a Potent Inhibitor of Heparin-amplified, FGF-2-induced FGFR-1 and Erk2 Kinase Activities and Subsequent Mitogenicity-- Because 6- O-desulfated heparin binds to FGF-2 but only weakly to the receptor (see Fig.  4,  A and  C), it may block formation of the ternary FGF-2-heparin-FGFR-1 complex.	bind
33974	2	8553	5	13	NULL	NULL	NULL	Heparin	Chemical		amplify					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24653_s_180	10816596	6-O-Desulfated Heparin Is a Potent Inhibitor of Heparin-amplified, FGF-2-induced FGFR-1 and Erk2 Kinase Activities and Subsequent Mitogenicity-- Because 6- O-desulfated heparin binds to FGF-2 but only weakly to the receptor (see Fig.  4,  A and  C), it may block formation of the ternary FGF-2-heparin-FGFR-1 complex.	bind
33975	3	8553	5	13	NULL	NULL	NULL	6- O-desulfated heparin	Chemical		inhibits		potentially			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24653_s_180	10816596	6-O-Desulfated Heparin Is a Potent Inhibitor of Heparin-amplified, FGF-2-induced FGFR-1 and Erk2 Kinase Activities and Subsequent Mitogenicity-- Because 6- O-desulfated heparin binds to FGF-2 but only weakly to the receptor (see Fig.  4,  A and  C), it may block formation of the ternary FGF-2-heparin-FGFR-1 complex.	bind
33976	4	8553	5	13	NULL	NULL	NULL	FGF-2	GP		induces					Erk2	GP	kinase activities of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24653_s_180	10816596	6-O-Desulfated Heparin Is a Potent Inhibitor of Heparin-amplified, FGF-2-induced FGFR-1 and Erk2 Kinase Activities and Subsequent Mitogenicity-- Because 6- O-desulfated heparin binds to FGF-2 but only weakly to the receptor (see Fig.  4,  A and  C), it may block formation of the ternary FGF-2-heparin-FGFR-1 complex.	bind
33977	5	8553	5	13	NULL	NULL	NULL	Heparin	Chemical		amplify					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24653_s_180	10816596	6-O-Desulfated Heparin Is a Potent Inhibitor of Heparin-amplified, FGF-2-induced FGFR-1 and Erk2 Kinase Activities and Subsequent Mitogenicity-- Because 6- O-desulfated heparin binds to FGF-2 but only weakly to the receptor (see Fig.  4,  A and  C), it may block formation of the ternary FGF-2-heparin-FGFR-1 complex.	bind
33978	6	8553	5	13	NULL	NULL	NULL	6- O-desulfated heparin	Chemical		inhibits		potentially			statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24653_s_180	10816596	6-O-Desulfated Heparin Is a Potent Inhibitor of Heparin-amplified, FGF-2-induced FGFR-1 and Erk2 Kinase Activities and Subsequent Mitogenicity-- Because 6- O-desulfated heparin binds to FGF-2 but only weakly to the receptor (see Fig.  4,  A and  C), it may block formation of the ternary FGF-2-heparin-FGFR-1 complex.	bind
33979	7	8553	5	13	NULL	NULL	NULL	6-O-Desulfated Heparin	Chemical		inhibits					mitogenicity	Process	subsequent			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24653_s_180	10816596	6-O-Desulfated Heparin Is a Potent Inhibitor of Heparin-amplified, FGF-2-induced FGFR-1 and Erk2 Kinase Activities and Subsequent Mitogenicity-- Because 6- O-desulfated heparin binds to FGF-2 but only weakly to the receptor (see Fig.  4,  A and  C), it may block formation of the ternary FGF-2-heparin-FGFR-1 complex.	bind
33980	8	8553	5	13	NULL	NULL	NULL	6- O-desulfated heparin	Chemical		bind					FGF-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24653_s_180	10816596	6-O-Desulfated Heparin Is a Potent Inhibitor of Heparin-amplified, FGF-2-induced FGFR-1 and Erk2 Kinase Activities and Subsequent Mitogenicity-- Because 6- O-desulfated heparin binds to FGF-2 but only weakly to the receptor (see Fig.  4,  A and  C), it may block formation of the ternary FGF-2-heparin-FGFR-1 complex.	bind
33981	9	8553	5	13	NULL	NULL	NULL	6- O-desulfated heparin	Chemical		bind		weakly			receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24653_s_180	10816596	6-O-Desulfated Heparin Is a Potent Inhibitor of Heparin-amplified, FGF-2-induced FGFR-1 and Erk2 Kinase Activities and Subsequent Mitogenicity-- Because 6- O-desulfated heparin binds to FGF-2 but only weakly to the receptor (see Fig.  4,  A and  C), it may block formation of the ternary FGF-2-heparin-FGFR-1 complex.	bind
33982	10	8553	5	13	NULL	NULL	NULL	6- O-desulfated heparin	Chemical		blocks					ternary FGF-2-heparin-FGFR-1 complex	GP	formation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24653_s_180	10816596	6-O-Desulfated Heparin Is a Potent Inhibitor of Heparin-amplified, FGF-2-induced FGFR-1 and Erk2 Kinase Activities and Subsequent Mitogenicity-- Because 6- O-desulfated heparin binds to FGF-2 but only weakly to the receptor (see Fig.  4,  A and  C), it may block formation of the ternary FGF-2-heparin-FGFR-1 complex.	bind
35479	1	8553	7	NULL	NULL	0	NULL	Heparin	NULL		amplify	NULL				FGFR- 1 activity	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24653_s_180	10816596	6-O-Desulfated Heparin Is a Potent Inhibitor of Heparin-amplified, FGF-2-induced FGFR-1 and Erk2 Kinase Activities and Subsequent Mitogenicity-- Because 6- O-desulfated heparin binds to FGF-2 but only weakly to the receptor (see Fig.  4,  A and  C), it may block formation of the ternary FGF-2-heparin-FGFR-1 complex.	bind
35480	2	8553	7	NULL	NULL	0	NULL	Heparin	NULL		amplify	NULL				Erk2 Kinase Activity	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24653_s_180	10816596	6-O-Desulfated Heparin Is a Potent Inhibitor of Heparin-amplified, FGF-2-induced FGFR-1 and Erk2 Kinase Activities and Subsequent Mitogenicity-- Because 6- O-desulfated heparin binds to FGF-2 but only weakly to the receptor (see Fig.  4,  A and  C), it may block formation of the ternary FGF-2-heparin-FGFR-1 complex.	bind
35482	3	8553	7	NULL	NULL	0	NULL	FGF-2	NULL		induce	NULL				FGFR-1 activity	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24653_s_180	10816596	6-O-Desulfated Heparin Is a Potent Inhibitor of Heparin-amplified, FGF-2-induced FGFR-1 and Erk2 Kinase Activities and Subsequent Mitogenicity-- Because 6- O-desulfated heparin binds to FGF-2 but only weakly to the receptor (see Fig.  4,  A and  C), it may block formation of the ternary FGF-2-heparin-FGFR-1 complex.	bind
35483	4	8553	7	NULL	NULL	0	NULL	FGF-2	NULL		induce	NULL				Erk2 Kinase Activity	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24653_s_180	10816596	6-O-Desulfated Heparin Is a Potent Inhibitor of Heparin-amplified, FGF-2-induced FGFR-1 and Erk2 Kinase Activities and Subsequent Mitogenicity-- Because 6- O-desulfated heparin binds to FGF-2 but only weakly to the receptor (see Fig.  4,  A and  C), it may block formation of the ternary FGF-2-heparin-FGFR-1 complex.	bind
35484	5	8553	7	NULL	NULL	0	NULL	6-O-Desulfated Heparin	NULL		inhibits	NULL	potently			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24653_s_180	10816596	6-O-Desulfated Heparin Is a Potent Inhibitor of Heparin-amplified, FGF-2-induced FGFR-1 and Erk2 Kinase Activities and Subsequent Mitogenicity-- Because 6- O-desulfated heparin binds to FGF-2 but only weakly to the receptor (see Fig.  4,  A and  C), it may block formation of the ternary FGF-2-heparin-FGFR-1 complex.	bind
35485	6	8553	7	NULL	NULL	0	NULL	6-O-Desulfated Heparin	NULL		inhibits	NULL	potently			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24653_s_180	10816596	6-O-Desulfated Heparin Is a Potent Inhibitor of Heparin-amplified, FGF-2-induced FGFR-1 and Erk2 Kinase Activities and Subsequent Mitogenicity-- Because 6- O-desulfated heparin binds to FGF-2 but only weakly to the receptor (see Fig.  4,  A and  C), it may block formation of the ternary FGF-2-heparin-FGFR-1 complex.	bind
35486	7	8553	7	NULL	NULL	0	NULL	6-O-Desulfated Heparin	NULL		inhibits	NULL	potently			statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24653_s_180	10816596	6-O-Desulfated Heparin Is a Potent Inhibitor of Heparin-amplified, FGF-2-induced FGFR-1 and Erk2 Kinase Activities and Subsequent Mitogenicity-- Because 6- O-desulfated heparin binds to FGF-2 but only weakly to the receptor (see Fig.  4,  A and  C), it may block formation of the ternary FGF-2-heparin-FGFR-1 complex.	bind
35487	8	8553	7	NULL	NULL	0	NULL	6-O-Desulfated Heparin	NULL		inhibits	NULL	potently			statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24653_s_180	10816596	6-O-Desulfated Heparin Is a Potent Inhibitor of Heparin-amplified, FGF-2-induced FGFR-1 and Erk2 Kinase Activities and Subsequent Mitogenicity-- Because 6- O-desulfated heparin binds to FGF-2 but only weakly to the receptor (see Fig.  4,  A and  C), it may block formation of the ternary FGF-2-heparin-FGFR-1 complex.	bind
35488	9	8553	7	NULL	NULL	0	NULL	6- O-desulfated heparin 	NULL		binds to	NULL				FGF-2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24653_s_180	10816596	6-O-Desulfated Heparin Is a Potent Inhibitor of Heparin-amplified, FGF-2-induced FGFR-1 and Erk2 Kinase Activities and Subsequent Mitogenicity-- Because 6- O-desulfated heparin binds to FGF-2 but only weakly to the receptor (see Fig.  4,  A and  C), it may block formation of the ternary FGF-2-heparin-FGFR-1 complex.	bind
35489	10	8553	7	NULL	NULL	0	NULL	Heparin	NULL		amplify	NULL				mitogenicity	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24653_s_180	10816596	6-O-Desulfated Heparin Is a Potent Inhibitor of Heparin-amplified, FGF-2-induced FGFR-1 and Erk2 Kinase Activities and Subsequent Mitogenicity-- Because 6- O-desulfated heparin binds to FGF-2 but only weakly to the receptor (see Fig.  4,  A and  C), it may block formation of the ternary FGF-2-heparin-FGFR-1 complex.	bind
35490	11	8553	7	NULL	NULL	0	NULL	FGF-2	NULL		induce	NULL				mitogenicity	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24653_s_180	10816596	6-O-Desulfated Heparin Is a Potent Inhibitor of Heparin-amplified, FGF-2-induced FGFR-1 and Erk2 Kinase Activities and Subsequent Mitogenicity-- Because 6- O-desulfated heparin binds to FGF-2 but only weakly to the receptor (see Fig.  4,  A and  C), it may block formation of the ternary FGF-2-heparin-FGFR-1 complex.	bind
35491	12	8553	7	NULL	NULL	0	NULL	6- O-desulfated heparin	NULL		binds 	NULL	weakly			receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24653_s_180	10816596	6-O-Desulfated Heparin Is a Potent Inhibitor of Heparin-amplified, FGF-2-induced FGFR-1 and Erk2 Kinase Activities and Subsequent Mitogenicity-- Because 6- O-desulfated heparin binds to FGF-2 but only weakly to the receptor (see Fig.  4,  A and  C), it may block formation of the ternary FGF-2-heparin-FGFR-1 complex.	bind
35492	13	8553	7	NULL	NULL	0	NULL	statement 9	NULL		blocks	NULL				ternary FGF-2-heparin-FGFR-1 complex	NULL	 formation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24653_s_180	10816596	6-O-Desulfated Heparin Is a Potent Inhibitor of Heparin-amplified, FGF-2-induced FGFR-1 and Erk2 Kinase Activities and Subsequent Mitogenicity-- Because 6- O-desulfated heparin binds to FGF-2 but only weakly to the receptor (see Fig.  4,  A and  C), it may block formation of the ternary FGF-2-heparin-FGFR-1 complex.	bind
35493	14	8553	7	NULL	NULL	0	NULL	statement 12	NULL		blocks	NULL				ternary FGF-2-heparin-FGFR-1 complex	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24653_s_180	10816596	6-O-Desulfated Heparin Is a Potent Inhibitor of Heparin-amplified, FGF-2-induced FGFR-1 and Erk2 Kinase Activities and Subsequent Mitogenicity-- Because 6- O-desulfated heparin binds to FGF-2 but only weakly to the receptor (see Fig.  4,  A and  C), it may block formation of the ternary FGF-2-heparin-FGFR-1 complex.	bind
33983	1	8554	5	13	NULL	NULL	NULL	6-Thiocyanato-FAD	Chemical		bind					DT-diaphorase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_6_2512_s_124	7531691	6-Thiocyanato-FAD binds  to DT-diaphorase with an absorption maximum at 441 nm.	bind
35494	1	8554	7	NULL	NULL	0	NULL	6-Thiocyanato-FAD	NULL		binds to	NULL				DT-diaphorase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_6_2512_s_124	7531691	6-Thiocyanato-FAD binds  to DT-diaphorase with an absorption maximum at 441 nm.	bind
33984	1	8555	5	13	NULL	NULL	NULL	apobec-1	GP		bind					apo B RNA	NucleicAcid	mammalian			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1772_s_475	11292850	60       Anant,S., MacGinnitie,A.J. and Davidson,N.O. (1995) The binding of apobec-1 to mammalian apo B RNA is stabilized by the presence of complementation factors which are required for post-transcriptional editing.	bind
33985	2	8555	5	13	NULL	NULL	NULL	statement 1	Process		stabilized by					complementation factors	GP	presence of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1772_s_475	11292850	60       Anant,S., MacGinnitie,A.J. and Davidson,N.O. (1995) The binding of apobec-1 to mammalian apo B RNA is stabilized by the presence of complementation factors which are required for post-transcriptional editing.	bind
33986	3	8555	5	13	NULL	NULL	NULL	complementation factors	GP		is required for					post-transcriptional editing	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1772_s_475	11292850	60       Anant,S., MacGinnitie,A.J. and Davidson,N.O. (1995) The binding of apobec-1 to mammalian apo B RNA is stabilized by the presence of complementation factors which are required for post-transcriptional editing.	bind
35495	1	8555	7	NULL	NULL	0	NULL	apobec-1	NULL		binds	NULL				apo B RNA	NULL	mammalian			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1772_s_475	11292850	60       Anant,S., MacGinnitie,A.J. and Davidson,N.O. (1995) The binding of apobec-1 to mammalian apo B RNA is stabilized by the presence of complementation factors which are required for post-transcriptional editing.	bind
35496	2	8555	7	NULL	NULL	0	NULL	complementation factors	NULL		stabilize	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1772_s_475	11292850	60       Anant,S., MacGinnitie,A.J. and Davidson,N.O. (1995) The binding of apobec-1 to mammalian apo B RNA is stabilized by the presence of complementation factors which are required for post-transcriptional editing.	bind
35497	3	8555	7	NULL	NULL	0	NULL	complementation factors	NULL		is required for	NULL				post-transcriptional editing	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1772_s_475	11292850	60       Anant,S., MacGinnitie,A.J. and Davidson,N.O. (1995) The binding of apobec-1 to mammalian apo B RNA is stabilized by the presence of complementation factors which are required for post-transcriptional editing.	bind
33987	1	8556	5	13	NULL	NULL	NULL	[1,2-13C]acetyl-CoA	Chemical		bind					HMG-CoA synthase	GP	wild-type			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_24_17946_s_256	10748155	600-MHz 1H,13C (omega2) half-filtered spectra of [1,2-13C]acetyl-CoA binding to wild type  HMG-CoA  synthase.	bind
35499	1	8556	7	NULL	NULL	0	NULL	[1,2-13C]acetyl-CoA	NULL		bind	NULL				HMG-CoA synthase	NULL	wild type			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_24_17946_s_256	10748155	600-MHz 1H,13C (omega2) half-filtered spectra of [1,2-13C]acetyl-CoA binding to wild type  HMG-CoA  synthase.	bind
33988	1	8557	5	13	NULL	NULL	NULL	60bca	GP		is					murine monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_11_5357_s_186	9784544	60bca is a murine monoclonal antibody that binds to CD14 and blocks LPS-CD14 interaction.	bind
33989	2	8557	5	13	NULL	NULL	NULL	60bca	GP		bind					CD14	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_11_5357_s_186	9784544	60bca is a murine monoclonal antibody that binds to CD14 and blocks LPS-CD14 interaction.	bind
33990	3	8557	5	13	NULL	NULL	NULL	LPS	Chemical		interacts with					CD14	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_11_5357_s_186	9784544	60bca is a murine monoclonal antibody that binds to CD14 and blocks LPS-CD14 interaction.	bind
33991	4	8557	5	13	NULL	NULL	NULL	statement 2	Process		blocks					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_11_5357_s_186	9784544	60bca is a murine monoclonal antibody that binds to CD14 and blocks LPS-CD14 interaction.	bind
35500	1	8557	7	NULL	NULL	0	NULL	60bca	NULL		is a type of	NULL				murine monoclonal antibody	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_11_5357_s_186	9784544	60bca is a murine monoclonal antibody that binds to CD14 and blocks LPS-CD14 interaction.	bind
35501	2	8557	7	NULL	NULL	0	NULL	60bca	NULL		binds to	NULL				CD14	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_11_5357_s_186	9784544	60bca is a murine monoclonal antibody that binds to CD14 and blocks LPS-CD14 interaction.	bind
35502	3	8557	7	NULL	NULL	0	NULL	LPS	NULL		interacts with	NULL				CD14	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_11_5357_s_186	9784544	60bca is a murine monoclonal antibody that binds to CD14 and blocks LPS-CD14 interaction.	bind
35503	4	8557	7	NULL	NULL	0	NULL	60bca	NULL		blocks	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_11_5357_s_186	9784544	60bca is a murine monoclonal antibody that binds to CD14 and blocks LPS-CD14 interaction.	bind
33992	1	8558	5	13	NULL	NULL	NULL	XPG	GP		is a type of					DNA repair endonuclease	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_3123_s_478	11452038	61       Gary,R., Ludwig,D.L., Cornelius,H.L., MacInnes,M.A. and Park,M.S. (1997) The DNA repair endonuclease XPG binds to proliferating cell nuclear antigen (PCNA) and shares sequence elements with the PCNA-binding regions of FEN-1 and cyclin-dependent kinase inhibitor p21.	bind
33993	2	8558	5	13	NULL	NULL	NULL	PCNA	GP		is					proliferating cell nuclear antigen	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_3123_s_478	11452038	61       Gary,R., Ludwig,D.L., Cornelius,H.L., MacInnes,M.A. and Park,M.S. (1997) The DNA repair endonuclease XPG binds to proliferating cell nuclear antigen (PCNA) and shares sequence elements with the PCNA-binding regions of FEN-1 and cyclin-dependent kinase inhibitor p21.	bind
33994	3	8558	5	13	NULL	NULL	NULL	XPG	GP		bind					PCNA	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_3123_s_478	11452038	61       Gary,R., Ludwig,D.L., Cornelius,H.L., MacInnes,M.A. and Park,M.S. (1997) The DNA repair endonuclease XPG binds to proliferating cell nuclear antigen (PCNA) and shares sequence elements with the PCNA-binding regions of FEN-1 and cyclin-dependent kinase inhibitor p21.	bind
33995	4	8558	5	13	NULL	NULL	NULL	XPG	GP		shares					FEN-1	GP	sequence elements with	PCNA-binding regions		NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_3123_s_478	11452038	61       Gary,R., Ludwig,D.L., Cornelius,H.L., MacInnes,M.A. and Park,M.S. (1997) The DNA repair endonuclease XPG binds to proliferating cell nuclear antigen (PCNA) and shares sequence elements with the PCNA-binding regions of FEN-1 and cyclin-dependent kinase inhibitor p21.	bind
33996	5	8558	5	13	NULL	NULL	NULL	XPG	GP		shares					p21	GP	sequence elements with			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_3123_s_478	11452038	61       Gary,R., Ludwig,D.L., Cornelius,H.L., MacInnes,M.A. and Park,M.S. (1997) The DNA repair endonuclease XPG binds to proliferating cell nuclear antigen (PCNA) and shares sequence elements with the PCNA-binding regions of FEN-1 and cyclin-dependent kinase inhibitor p21.	bind
33997	6	8558	5	13	NULL	NULL	NULL	p21	GP		is a type of					cyclin-dependent kinase inhibitor	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_3123_s_478	11452038	61       Gary,R., Ludwig,D.L., Cornelius,H.L., MacInnes,M.A. and Park,M.S. (1997) The DNA repair endonuclease XPG binds to proliferating cell nuclear antigen (PCNA) and shares sequence elements with the PCNA-binding regions of FEN-1 and cyclin-dependent kinase inhibitor p21.	bind
35504	1	8558	7	NULL	NULL	0	NULL	XPG	NULL		binds to	NULL				PCNA	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_3123_s_478	11452038	61       Gary,R., Ludwig,D.L., Cornelius,H.L., MacInnes,M.A. and Park,M.S. (1997) The DNA repair endonuclease XPG binds to proliferating cell nuclear antigen (PCNA) and shares sequence elements with the PCNA-binding regions of FEN-1 and cyclin-dependent kinase inhibitor p21.	bind
35505	2	8558	7	NULL	NULL	0	NULL	XPG	NULL		is a type of	NULL				DNA repair endonuclease	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_3123_s_478	11452038	61       Gary,R., Ludwig,D.L., Cornelius,H.L., MacInnes,M.A. and Park,M.S. (1997) The DNA repair endonuclease XPG binds to proliferating cell nuclear antigen (PCNA) and shares sequence elements with the PCNA-binding regions of FEN-1 and cyclin-dependent kinase inhibitor p21.	bind
35506	3	8558	7	NULL	NULL	0	NULL	PCNA	NULL		is	NULL				proliferating cell nuclear antigen	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_3123_s_478	11452038	61       Gary,R., Ludwig,D.L., Cornelius,H.L., MacInnes,M.A. and Park,M.S. (1997) The DNA repair endonuclease XPG binds to proliferating cell nuclear antigen (PCNA) and shares sequence elements with the PCNA-binding regions of FEN-1 and cyclin-dependent kinase inhibitor p21.	bind
35507	4	8558	7	NULL	NULL	0	NULL	XPG	NULL		shares	NULL				FEN-1	NULL	sequence elements with	PCNA-binding regions of 		NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_3123_s_478	11452038	61       Gary,R., Ludwig,D.L., Cornelius,H.L., MacInnes,M.A. and Park,M.S. (1997) The DNA repair endonuclease XPG binds to proliferating cell nuclear antigen (PCNA) and shares sequence elements with the PCNA-binding regions of FEN-1 and cyclin-dependent kinase inhibitor p21.	bind
35508	5	8558	7	NULL	NULL	0	NULL	p21	NULL		is a type of	NULL				cyclin-dependent kinase inhibitor	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_3123_s_478	11452038	61       Gary,R., Ludwig,D.L., Cornelius,H.L., MacInnes,M.A. and Park,M.S. (1997) The DNA repair endonuclease XPG binds to proliferating cell nuclear antigen (PCNA) and shares sequence elements with the PCNA-binding regions of FEN-1 and cyclin-dependent kinase inhibitor p21.	bind
35509	6	8558	7	NULL	NULL	0	NULL	XPG	NULL		shares	NULL				p21	NULL	sequence elements with	PCNA-binding regions of		NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_3123_s_478	11452038	61       Gary,R., Ludwig,D.L., Cornelius,H.L., MacInnes,M.A. and Park,M.S. (1997) The DNA repair endonuclease XPG binds to proliferating cell nuclear antigen (PCNA) and shares sequence elements with the PCNA-binding regions of FEN-1 and cyclin-dependent kinase inhibitor p21.	bind
35510	1	8559	7	NULL	NULL	0	NULL	U2 snRNP	NULL		bind	NULL				pre-mRNA	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1741_s_406	11292847	61       Ruby,S.W., Chang,T.-H. and Abelson,J. (1993) Four yeast spliceosomal proteins (PRP5, PRP9, PRP11, and PRP21) interact to promote U2 snRNP binding to pre-mRNA.	bind
35511	2	8559	7	NULL	NULL	0	NULL	PRP5	NULL		promote	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1741_s_406	11292847	61       Ruby,S.W., Chang,T.-H. and Abelson,J. (1993) Four yeast spliceosomal proteins (PRP5, PRP9, PRP11, and PRP21) interact to promote U2 snRNP binding to pre-mRNA.	bind
35512	3	8559	7	NULL	NULL	0	NULL	PRP9	NULL		promote	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1741_s_406	11292847	61       Ruby,S.W., Chang,T.-H. and Abelson,J. (1993) Four yeast spliceosomal proteins (PRP5, PRP9, PRP11, and PRP21) interact to promote U2 snRNP binding to pre-mRNA.	bind
35513	4	8559	7	NULL	NULL	0	NULL	PRP11	NULL		promote	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1741_s_406	11292847	61       Ruby,S.W., Chang,T.-H. and Abelson,J. (1993) Four yeast spliceosomal proteins (PRP5, PRP9, PRP11, and PRP21) interact to promote U2 snRNP binding to pre-mRNA.	bind
35514	5	8559	7	NULL	NULL	0	NULL	PRP21	NULL		promote	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1741_s_406	11292847	61       Ruby,S.W., Chang,T.-H. and Abelson,J. (1993) Four yeast spliceosomal proteins (PRP5, PRP9, PRP11, and PRP21) interact to promote U2 snRNP binding to pre-mRNA.	bind
35515	6	8559	7	NULL	NULL	0	NULL	PRP5	NULL		is a type of	NULL				yeast spliceosomal protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1741_s_406	11292847	61       Ruby,S.W., Chang,T.-H. and Abelson,J. (1993) Four yeast spliceosomal proteins (PRP5, PRP9, PRP11, and PRP21) interact to promote U2 snRNP binding to pre-mRNA.	bind
35516	7	8559	7	NULL	NULL	0	NULL	PRP9	NULL		is a type of	NULL				yeast spliceosomal protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1741_s_406	11292847	61       Ruby,S.W., Chang,T.-H. and Abelson,J. (1993) Four yeast spliceosomal proteins (PRP5, PRP9, PRP11, and PRP21) interact to promote U2 snRNP binding to pre-mRNA.	bind
35517	8	8559	7	NULL	NULL	0	NULL	PRP11	NULL		is a type of	NULL				yeast spliceosomal protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1741_s_406	11292847	61       Ruby,S.W., Chang,T.-H. and Abelson,J. (1993) Four yeast spliceosomal proteins (PRP5, PRP9, PRP11, and PRP21) interact to promote U2 snRNP binding to pre-mRNA.	bind
35518	9	8559	7	NULL	NULL	0	NULL	 PRP21	NULL		is a type of	NULL				yeast spliceosomal protein	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1741_s_406	11292847	61       Ruby,S.W., Chang,T.-H. and Abelson,J. (1993) Four yeast spliceosomal proteins (PRP5, PRP9, PRP11, and PRP21) interact to promote U2 snRNP binding to pre-mRNA.	bind
34296	1	8560	5	13	NULL	NULL	NULL	angiotensin II	GP		upregulates					SM alpha-actin	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_2_221_s_248	10666419	61  Interestingly, in previous studies, we found that when the "`weak"' SM alpha-actin CArGs were replaced with the much stronger SRE CArG, promoter activity increased dramatically and was no longer limited to SMCs. 48  In addition, we presented evidence indicating that angiotensin II - induced upregulation of SM alpha-actin expression was mediated by increased expression of the homeodomain protein, Mhox, which increased SRF binding to CArG B. 61  Importantly, Mhox itself was not found within the SRF-containing gel-shift complexes and could not account for the SMC SRF-containing higher order complex.	bind
34299	2	8560	5	13	NULL	NULL	NULL	Mhox	GP	increased expression of	increases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_2_221_s_248	10666419	61  Interestingly, in previous studies, we found that when the "`weak"' SM alpha-actin CArGs were replaced with the much stronger SRE CArG, promoter activity increased dramatically and was no longer limited to SMCs. 48  In addition, we presented evidence indicating that angiotensin II - induced upregulation of SM alpha-actin expression was mediated by increased expression of the homeodomain protein, Mhox, which increased SRF binding to CArG B. 61  Importantly, Mhox itself was not found within the SRF-containing gel-shift complexes and could not account for the SMC SRF-containing higher order complex.	bind
34301	3	8560	5	13	NULL	NULL	NULL	Mhox	GP		is a type of					homeodomain protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_2_221_s_248	10666419	61  Interestingly, in previous studies, we found that when the "`weak"' SM alpha-actin CArGs were replaced with the much stronger SRE CArG, promoter activity increased dramatically and was no longer limited to SMCs. 48  In addition, we presented evidence indicating that angiotensin II - induced upregulation of SM alpha-actin expression was mediated by increased expression of the homeodomain protein, Mhox, which increased SRF binding to CArG B. 61  Importantly, Mhox itself was not found within the SRF-containing gel-shift complexes and could not account for the SMC SRF-containing higher order complex.	bind
34302	4	8560	5	13	NULL	NULL	NULL	SRF	GP		bind									CArG B	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_2_221_s_248	10666419	61  Interestingly, in previous studies, we found that when the "`weak"' SM alpha-actin CArGs were replaced with the much stronger SRE CArG, promoter activity increased dramatically and was no longer limited to SMCs. 48  In addition, we presented evidence indicating that angiotensin II - induced upregulation of SM alpha-actin expression was mediated by increased expression of the homeodomain protein, Mhox, which increased SRF binding to CArG B. 61  Importantly, Mhox itself was not found within the SRF-containing gel-shift complexes and could not account for the SMC SRF-containing higher order complex.	bind
34303	5	8560	5	13	NULL	NULL	NULL	Mhox	GP		increases					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_2_221_s_248	10666419	61  Interestingly, in previous studies, we found that when the "`weak"' SM alpha-actin CArGs were replaced with the much stronger SRE CArG, promoter activity increased dramatically and was no longer limited to SMCs. 48  In addition, we presented evidence indicating that angiotensin II - induced upregulation of SM alpha-actin expression was mediated by increased expression of the homeodomain protein, Mhox, which increased SRF binding to CArG B. 61  Importantly, Mhox itself was not found within the SRF-containing gel-shift complexes and could not account for the SMC SRF-containing higher order complex.	bind
35528	1	8560	7	10	NULL	0	NULL	angiotensin II			upregulates					SM alpha-actin expression		expression of 			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_2_221_s_248	10666419	61  Interestingly, in previous studies, we found that when the "`weak"' SM alpha-actin CArGs were replaced with the much stronger SRE CArG, promoter activity increased dramatically and was no longer limited to SMCs. 48  In addition, we presented evidence indicating that angiotensin II - induced upregulation of SM alpha-actin expression was mediated by increased expression of the homeodomain protein, Mhox, which increased SRF binding to CArG B. 61  Importantly, Mhox itself was not found within the SRF-containing gel-shift complexes and could not account for the SMC SRF-containing higher order complex.	bind
35533	2	8560	7	NULL	NULL	0	NULL	Mhox	NULL	expression of	increase	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_86_2_221_s_248	10666419	61  Interestingly, in previous studies, we found that when the "`weak"' SM alpha-actin CArGs were replaced with the much stronger SRE CArG, promoter activity increased dramatically and was no longer limited to SMCs. 48  In addition, we presented evidence indicating that angiotensin II - induced upregulation of SM alpha-actin expression was mediated by increased expression of the homeodomain protein, Mhox, which increased SRF binding to CArG B. 61  Importantly, Mhox itself was not found within the SRF-containing gel-shift complexes and could not account for the SMC SRF-containing higher order complex.	bind
35540	3	8560	7	NULL	NULL	0	NULL	Mhox	NULL		is a type of	NULL				homeodomain protein	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_86_2_221_s_248	10666419	61  Interestingly, in previous studies, we found that when the "`weak"' SM alpha-actin CArGs were replaced with the much stronger SRE CArG, promoter activity increased dramatically and was no longer limited to SMCs. 48  In addition, we presented evidence indicating that angiotensin II - induced upregulation of SM alpha-actin expression was mediated by increased expression of the homeodomain protein, Mhox, which increased SRF binding to CArG B. 61  Importantly, Mhox itself was not found within the SRF-containing gel-shift complexes and could not account for the SMC SRF-containing higher order complex.	bind
35541	4	8560	7	NULL	NULL	0	NULL	SRF	NULL		bind	NULL					NULL			CArG B	NULL		0	NULL	NULL	NULL	gw60_circulationres_86_2_221_s_248	10666419	61  Interestingly, in previous studies, we found that when the "`weak"' SM alpha-actin CArGs were replaced with the much stronger SRE CArG, promoter activity increased dramatically and was no longer limited to SMCs. 48  In addition, we presented evidence indicating that angiotensin II - induced upregulation of SM alpha-actin expression was mediated by increased expression of the homeodomain protein, Mhox, which increased SRF binding to CArG B. 61  Importantly, Mhox itself was not found within the SRF-containing gel-shift complexes and could not account for the SMC SRF-containing higher order complex.	bind
35542	5	8560	7	NULL	NULL	0	NULL	Mhox	NULL		increase	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_86_2_221_s_248	10666419	61  Interestingly, in previous studies, we found that when the "`weak"' SM alpha-actin CArGs were replaced with the much stronger SRE CArG, promoter activity increased dramatically and was no longer limited to SMCs. 48  In addition, we presented evidence indicating that angiotensin II - induced upregulation of SM alpha-actin expression was mediated by increased expression of the homeodomain protein, Mhox, which increased SRF binding to CArG B. 61  Importantly, Mhox itself was not found within the SRF-containing gel-shift complexes and could not account for the SMC SRF-containing higher order complex.	bind
33999	1	8561	5	13	NULL	NULL	NULL	collagen	GP		bind					GPVI	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_1_14_s_144	11788455	61 -  63 Collagen binding to GPVI induces platelet activation through a pathway that involves phosphorylation of the FcRgamma chain followed by the binding of Syk and the phosphorylation-dependent activation of PLCgamma2.	bind
34000	2	8561	5	13	NULL	NULL	NULL	statement 1	Process		induces					platelet	Cell	activation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_1_14_s_144	11788455	61 -  63 Collagen binding to GPVI induces platelet activation through a pathway that involves phosphorylation of the FcRgamma chain followed by the binding of Syk and the phosphorylation-dependent activation of PLCgamma2.	bind
34001	3	8561	5	13	NULL	NULL	NULL	statement 2	Process		occurs through					pathway	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_1_14_s_144	11788455	61 -  63 Collagen binding to GPVI induces platelet activation through a pathway that involves phosphorylation of the FcRgamma chain followed by the binding of Syk and the phosphorylation-dependent activation of PLCgamma2.	bind
34002	4	8561	5	13	NULL	NULL	NULL	FcRgamma chain	GP	phosphorylation of	is followed by					Syk	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_1_14_s_144	11788455	61 -  63 Collagen binding to GPVI induces platelet activation through a pathway that involves phosphorylation of the FcRgamma chain followed by the binding of Syk and the phosphorylation-dependent activation of PLCgamma2.	bind
34003	5	8561	5	13	NULL	NULL	NULL	statement 3	Process		involves					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_1_14_s_144	11788455	61 -  63 Collagen binding to GPVI induces platelet activation through a pathway that involves phosphorylation of the FcRgamma chain followed by the binding of Syk and the phosphorylation-dependent activation of PLCgamma2.	bind
34004	6	8561	5	13	NULL	NULL	NULL	PLCgamma2	GP	activation of	is dependent on					phosphorylation	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_1_14_s_144	11788455	61 -  63 Collagen binding to GPVI induces platelet activation through a pathway that involves phosphorylation of the FcRgamma chain followed by the binding of Syk and the phosphorylation-dependent activation of PLCgamma2.	bind
34005	7	8561	5	13	NULL	NULL	NULL	statement 3	Process		involves					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_1_14_s_144	11788455	61 -  63 Collagen binding to GPVI induces platelet activation through a pathway that involves phosphorylation of the FcRgamma chain followed by the binding of Syk and the phosphorylation-dependent activation of PLCgamma2.	bind
35544	1	8561	7	NULL	NULL	0	NULL	Collagen	NULL		bind	NULL				GPVI	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_1_14_s_144	11788455	61 -  63 Collagen binding to GPVI induces platelet activation through a pathway that involves phosphorylation of the FcRgamma chain followed by the binding of Syk and the phosphorylation-dependent activation of PLCgamma2.	bind
35545	2	8561	7	NULL	NULL	0	NULL	statement 1	NULL		induces	NULL				platelet	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_1_14_s_144	11788455	61 -  63 Collagen binding to GPVI induces platelet activation through a pathway that involves phosphorylation of the FcRgamma chain followed by the binding of Syk and the phosphorylation-dependent activation of PLCgamma2.	bind
35546	3	8561	7	NULL	NULL	0	NULL	statement 2	NULL		occurs through	NULL				FcRgamma chain	NULL	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_1_14_s_144	11788455	61 -  63 Collagen binding to GPVI induces platelet activation through a pathway that involves phosphorylation of the FcRgamma chain followed by the binding of Syk and the phosphorylation-dependent activation of PLCgamma2.	bind
35547	4	8561	7	NULL	NULL	0	NULL	statement 3	NULL		is followed by	NULL				Syk	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_1_14_s_144	11788455	61 -  63 Collagen binding to GPVI induces platelet activation through a pathway that involves phosphorylation of the FcRgamma chain followed by the binding of Syk and the phosphorylation-dependent activation of PLCgamma2.	bind
35548	5	8561	7	NULL	NULL	0	NULL	PLCgamma2	NULL	activation of	depends on	NULL				phosphorylation	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_1_14_s_144	11788455	61 -  63 Collagen binding to GPVI induces platelet activation through a pathway that involves phosphorylation of the FcRgamma chain followed by the binding of Syk and the phosphorylation-dependent activation of PLCgamma2.	bind
35549	6	8561	7	NULL	NULL	0	NULL	statement 3	NULL		is followed by	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_1_14_s_144	11788455	61 -  63 Collagen binding to GPVI induces platelet activation through a pathway that involves phosphorylation of the FcRgamma chain followed by the binding of Syk and the phosphorylation-dependent activation of PLCgamma2.	bind
34006	1	8562	5	13	NULL	NULL	NULL	Fas ligand	GP		induces					Fas	GP	conformational change in			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_80	15539639	61 - 63   Using the Fas death receptor as an example, the binding of Fas ligand is presumed to induce a conformational change in Fas.	bind
35550	1	8562	7	NULL	NULL	0	NULL	Fas ligand	NULL		induce	NULL				Fas	NULL	conformational change in			NULL		0	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_80	15539639	61 - 63   Using the Fas death receptor as an example, the binding of Fas ligand is presumed to induce a conformational change in Fas.	bind
34007	1	8563	5	13	NULL	NULL	NULL	C/EBPbeta	GP		bind					COX-2	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_127	15681294	61 Aspirin and sodium salicylate at 10 - 5 M selectively inhibited C/EBPbeta binding to COX-2 promoter without an effect on p50/RelA NF-kappaB binding.	bind
34008	2	8563	5	13	NULL	NULL	NULL	aspirin	Chemical		inhibits		selectively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_127	15681294	61 Aspirin and sodium salicylate at 10 - 5 M selectively inhibited C/EBPbeta binding to COX-2 promoter without an effect on p50/RelA NF-kappaB binding.	bind
34009	3	8563	5	13	NULL	NULL	NULL	sodium salicylate	Chemical		inhibits		selectively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_127	15681294	61 Aspirin and sodium salicylate at 10 - 5 M selectively inhibited C/EBPbeta binding to COX-2 promoter without an effect on p50/RelA NF-kappaB binding.	bind
34010	4	8563	5	13	NULL	NULL	NULL	p50/RelA	GP		bind					NF-kappaB	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_127	15681294	61 Aspirin and sodium salicylate at 10 - 5 M selectively inhibited C/EBPbeta binding to COX-2 promoter without an effect on p50/RelA NF-kappaB binding.	bind
34011	5	8563	5	13	NULL	NULL	NULL	aspirin	Chemical		does not effect					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_127	15681294	61 Aspirin and sodium salicylate at 10 - 5 M selectively inhibited C/EBPbeta binding to COX-2 promoter without an effect on p50/RelA NF-kappaB binding.	bind
34012	6	8563	5	13	NULL	NULL	NULL	sodium salicylate	Chemical		does not effect					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_127	15681294	61 Aspirin and sodium salicylate at 10 - 5 M selectively inhibited C/EBPbeta binding to COX-2 promoter without an effect on p50/RelA NF-kappaB binding.	bind
35551	1	8563	7	NULL	NULL	0	NULL	C/EBPbeta	NULL		bind	NULL				COX-2	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_127	15681294	61 Aspirin and sodium salicylate at 10 - 5 M selectively inhibited C/EBPbeta binding to COX-2 promoter without an effect on p50/RelA NF-kappaB binding.	bind
35552	2	8563	7	NULL	NULL	0	NULL	p50/RelA	NULL		bind	NULL				NF-kappaB	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_127	15681294	61 Aspirin and sodium salicylate at 10 - 5 M selectively inhibited C/EBPbeta binding to COX-2 promoter without an effect on p50/RelA NF-kappaB binding.	bind
35553	3	8563	7	NULL	NULL	0	NULL	 Aspirin	NULL		inhibits	NULL	selectively			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_127	15681294	61 Aspirin and sodium salicylate at 10 - 5 M selectively inhibited C/EBPbeta binding to COX-2 promoter without an effect on p50/RelA NF-kappaB binding.	bind
35554	4	8563	7	NULL	NULL	0	NULL	sodium salicylate	NULL		inhibits	NULL	selectively			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_127	15681294	61 Aspirin and sodium salicylate at 10 - 5 M selectively inhibited C/EBPbeta binding to COX-2 promoter without an effect on p50/RelA NF-kappaB binding.	bind
35555	5	8563	7	NULL	NULL	0	NULL	Aspirin	NULL		does not effect	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_127	15681294	61 Aspirin and sodium salicylate at 10 - 5 M selectively inhibited C/EBPbeta binding to COX-2 promoter without an effect on p50/RelA NF-kappaB binding.	bind
35556	6	8563	7	NULL	NULL	0	NULL	sodium salicylate	NULL		does not effect	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_679_s_127	15681294	61 Aspirin and sodium salicylate at 10 - 5 M selectively inhibited C/EBPbeta binding to COX-2 promoter without an effect on p50/RelA NF-kappaB binding.	bind
34013	1	8564	5	13	NULL	NULL	NULL	erythropoietin ligand	GP		bind					homodimeric erythropoietin receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_113_20_2454_s_92	16717164	61 Ligand binding of erythropoietin to the homodimeric erythropoietin receptor activates antiapoptotic signal transduction pathways.	bind
34014	2	8564	5	13	NULL	NULL	NULL	statement 1	Process		activates					antiapoptotic signal transduction pathways	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_113_20_2454_s_92	16717164	61 Ligand binding of erythropoietin to the homodimeric erythropoietin receptor activates antiapoptotic signal transduction pathways.	bind
35557	1	8564	7	NULL	NULL	0	NULL	erythropoietin	NULL		bind	NULL				homodimeric erythropoietin receptor	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulation_113_20_2454_s_92	16717164	61 Ligand binding of erythropoietin to the homodimeric erythropoietin receptor activates antiapoptotic signal transduction pathways.	bind
35558	2	8564	7	NULL	NULL	0	NULL	statement 1	NULL		activates	NULL				antiapoptotic signal transduction pathways	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_113_20_2454_s_92	16717164	61 Ligand binding of erythropoietin to the homodimeric erythropoietin receptor activates antiapoptotic signal transduction pathways.	bind
34015	1	8565	5	13	NULL	NULL	NULL	CD4+ cells	Cell		bind					ECM proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_157_4_1207_s_234	11021825	61- 64  Indeed, it has been reported that binding of CD4+ cells to ECM proteins, most likely through conformational changes resulting in better presentation to their receptor, may in turn enhance cytokine activity.	bind
35559	1	8565	7	NULL	NULL	0	NULL	CD4+ cells 	NULL		bind	NULL				ECM proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_157_4_1207_s_234	11021825	61- 64  Indeed, it has been reported that binding of CD4+ cells to ECM proteins, most likely through conformational changes resulting in better presentation to their receptor, may in turn enhance cytokine activity.	bind
34019	1	8566	5	13	NULL	NULL	NULL	heparin	Chemical		bind					Tat	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_5_3254_s_143	11024024	61-63), thus suggesting that heparin could compete with cell surface HS proteoglycans for binding to Tat, as observed for other heparin binding growth factors.	bind
34020	2	8566	5	13	NULL	NULL	NULL	HS proteoglycans	GP	cell surface	bind					Tat	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_5_3254_s_143	11024024	61-63), thus suggesting that heparin could compete with cell surface HS proteoglycans for binding to Tat, as observed for other heparin binding growth factors.	bind
34021	3	8566	5	13	NULL	NULL	NULL	statement 1	Process		competes with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_5_3254_s_143	11024024	61-63), thus suggesting that heparin could compete with cell surface HS proteoglycans for binding to Tat, as observed for other heparin binding growth factors.	bind
35564	1	8566	7	10	NULL	0	NULL	HS proteoglycans		cell surface	bind					Tat					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_5_3254_s_143	11024024	61-63), thus suggesting that heparin could compete with cell surface HS proteoglycans for binding to Tat, as observed for other heparin binding growth factors.	bind
35565	2	8566	7	NULL	NULL	0	NULL	heparin	NULL		bind	NULL				Tat	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_5_3254_s_143	11024024	61-63), thus suggesting that heparin could compete with cell surface HS proteoglycans for binding to Tat, as observed for other heparin binding growth factors.	bind
35566	3	8566	7	NULL	NULL	0	NULL	statement 2	NULL		compete with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_5_3254_s_143	11024024	61-63), thus suggesting that heparin could compete with cell surface HS proteoglycans for binding to Tat, as observed for other heparin binding growth factors.	bind
34022	1	8567	5	13	NULL	NULL	NULL	EBNA-1	GP		bind		sequence-specific			plasmid DNA	NucleicAcid			clustered sites in maintenance region	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_23_4881_s_495	11726698	62       Rawlins,D.R., Milman,G., Hayward,S.D. and Hayward,G.S. (1985) Sequence-specific DNA binding of the Epstein-Barr virus nuclear antigen (EBNA-1) to clustered sites in the plasmid maintenance region.	bind
34023	2	8567	5	13	NULL	NULL	NULL	EBNA-1	GP		is					Epstein-Barr virus nuclear antigen	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_23_4881_s_495	11726698	62       Rawlins,D.R., Milman,G., Hayward,S.D. and Hayward,G.S. (1985) Sequence-specific DNA binding of the Epstein-Barr virus nuclear antigen (EBNA-1) to clustered sites in the plasmid maintenance region.	bind
35568	1	8567	7	NULL	NULL	0	NULL	EBNA-1	NULL		bind	NULL	sequence-specific			plasmid DNA	NULL			clustered sites in the maintenance region	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_23_4881_s_495	11726698	62       Rawlins,D.R., Milman,G., Hayward,S.D. and Hayward,G.S. (1985) Sequence-specific DNA binding of the Epstein-Barr virus nuclear antigen (EBNA-1) to clustered sites in the plasmid maintenance region.	bind
35569	2	8567	7	NULL	NULL	0	NULL	EBNA-1	NULL		is	NULL				Epstein-Barr virus nuclear antigen	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_23_4881_s_495	11726698	62       Rawlins,D.R., Milman,G., Hayward,S.D. and Hayward,G.S. (1985) Sequence-specific DNA binding of the Epstein-Barr virus nuclear antigen (EBNA-1) to clustered sites in the plasmid maintenance region.	bind
34024	1	8568	5	13	NULL	NULL	NULL	FGF-2	GP		interacts with					FGFR	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_162_3_977_s_295	12598330	62  Thus the location of the HS sequences that bind to the FGFR, together with steric constraints may strongly influence the FGF-2 to FGFR interaction.	bind
34025	2	8568	5	13	NULL	NULL	NULL	HS sequences	GP		bind					FGFR	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_162_3_977_s_295	12598330	62  Thus the location of the HS sequences that bind to the FGFR, together with steric constraints may strongly influence the FGF-2 to FGFR interaction.	bind
34026	3	8568	5	13	NULL	NULL	NULL	statement 2	Process	location of	influence		strongly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_162_3_977_s_295	12598330	62  Thus the location of the HS sequences that bind to the FGFR, together with steric constraints may strongly influence the FGF-2 to FGFR interaction.	bind
34027	4	8568	5	13	NULL	NULL	NULL	steric constraints			influence		strongly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_162_3_977_s_295	12598330	62  Thus the location of the HS sequences that bind to the FGFR, together with steric constraints may strongly influence the FGF-2 to FGFR interaction.	bind
35570	1	8568	7	10	NULL	0	NULL	HS sequences	NULL		bind	NULL				FGFR	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_162_3_977_s_295	12598330	62  Thus the location of the HS sequences that bind to the FGFR, together with steric constraints may strongly influence the FGF-2 to FGFR interaction.	bind
35571	2	8568	7	NULL	NULL	0	NULL	FGF-2 	NULL		interacts with	NULL				FGFR	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_162_3_977_s_295	12598330	62  Thus the location of the HS sequences that bind to the FGFR, together with steric constraints may strongly influence the FGF-2 to FGFR interaction.	bind
35572	3	8568	7	NULL	NULL	0	NULL	steric constraints	NULL		influence	NULL	may strongly			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_162_3_977_s_295	12598330	62  Thus the location of the HS sequences that bind to the FGFR, together with steric constraints may strongly influence the FGF-2 to FGFR interaction.	bind
35573	4	8568	7	NULL	NULL	0	NULL	statement 1	NULL		influence	NULL	strongly			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_162_3_977_s_295	12598330	62  Thus the location of the HS sequences that bind to the FGFR, together with steric constraints may strongly influence the FGF-2 to FGFR interaction.	bind
34044	1	8569	5	13	NULL	NULL	NULL	EBNA1 protein	GP		bind		constitutively			Epstein-Barr virus	Organism			oriP	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_23_4881_s_498	11726698	63       Hsieh,D.J., Camiolo,S.M. and Yates,J.L. (1993) Constitutive binding of EBNA1 protein to the Epstein-Barr virus replication origin, oriP, with distortion of DNA structure during latent infection.	bind
34045	2	8569	5	13	NULL	NULL	NULL	oriP	NucleicAcid		is					replication origin	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_23_4881_s_498	11726698	63       Hsieh,D.J., Camiolo,S.M. and Yates,J.L. (1993) Constitutive binding of EBNA1 protein to the Epstein-Barr virus replication origin, oriP, with distortion of DNA structure during latent infection.	bind
35575	1	8569	7	10	NULL	0	NULL	EBNA1 protein 			binds		constitutively			Epstein-Barr virus				oriP	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_23_4881_s_498	11726698	63       Hsieh,D.J., Camiolo,S.M. and Yates,J.L. (1993) Constitutive binding of EBNA1 protein to the Epstein-Barr virus replication origin, oriP, with distortion of DNA structure during latent infection.	bind
35576	2	8569	7	NULL	NULL	0	NULL	oriP	NULL		is 	NULL				Epstein-Barr virus replication origin	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_23_4881_s_498	11726698	63       Hsieh,D.J., Camiolo,S.M. and Yates,J.L. (1993) Constitutive binding of EBNA1 protein to the Epstein-Barr virus replication origin, oriP, with distortion of DNA structure during latent infection.	bind
34047	1	8570	5	13	NULL	NULL	NULL	CCR3	GP		bind					eotaxin	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_6_1861_s_251	9846976	63  CCR3 was originally described as the receptor for eotaxin, but in the mouse CCR3 will bind MIP-1alpha.	bind
34048	2	8570	5	13	NULL	NULL	NULL	CCR3	GP		bind					MIP-1alpha	GP	mouse			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_6_1861_s_251	9846976	63  CCR3 was originally described as the receptor for eotaxin, but in the mouse CCR3 will bind MIP-1alpha.	bind
35577	1	8570	7	NULL	NULL	0	NULL	eotaxin	NULL		bind	NULL				CCR3 receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_6_1861_s_251	9846976	63  CCR3 was originally described as the receptor for eotaxin, but in the mouse CCR3 will bind MIP-1alpha.	bind
35578	2	8570	7	NULL	NULL	0	NULL	MIP-1alpha	NULL		bind	NULL				CCR3	NULL	mouse			NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_6_1861_s_251	9846976	63  CCR3 was originally described as the receptor for eotaxin, but in the mouse CCR3 will bind MIP-1alpha.	bind
34049	1	8571	5	13	NULL	NULL	NULL	cytochrome c	GP		bind					Apaf-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_6_2229_s_244	12466137	63  The cytochrome c is known to bind with the adaptor molecule Apaf-1 and form the apoptosome that activates caspase-9, a caspase that cleaves and activates caspase-3.	bind
34050	2	8571	5	13	NULL	NULL	NULL	Apaf-1	GP		is a type of					adaptor molecule	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_6_2229_s_244	12466137	63  The cytochrome c is known to bind with the adaptor molecule Apaf-1 and form the apoptosome that activates caspase-9, a caspase that cleaves and activates caspase-3.	bind
34051	3	8571	5	13	NULL	NULL	NULL	statement 1	Process		forms					apoptosome	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_6_2229_s_244	12466137	63  The cytochrome c is known to bind with the adaptor molecule Apaf-1 and form the apoptosome that activates caspase-9, a caspase that cleaves and activates caspase-3.	bind
34052	4	8571	5	13	NULL	NULL	NULL	apoptosome	GP		activates					caspase-9	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_6_2229_s_244	12466137	63  The cytochrome c is known to bind with the adaptor molecule Apaf-1 and form the apoptosome that activates caspase-9, a caspase that cleaves and activates caspase-3.	bind
34053	5	8571	5	13	NULL	NULL	NULL	caspase-9	GP		cleaves					caspase-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_6_2229_s_244	12466137	63  The cytochrome c is known to bind with the adaptor molecule Apaf-1 and form the apoptosome that activates caspase-9, a caspase that cleaves and activates caspase-3.	bind
34054	6	8571	5	13	NULL	NULL	NULL	statement 5	Process		activates					caspase-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_6_2229_s_244	12466137	63  The cytochrome c is known to bind with the adaptor molecule Apaf-1 and form the apoptosome that activates caspase-9, a caspase that cleaves and activates caspase-3.	bind
35579	1	8571	7	NULL	NULL	0	NULL	 cytochrome c	NULL		bind	NULL				Apaf-1	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_6_2229_s_244	12466137	63  The cytochrome c is known to bind with the adaptor molecule Apaf-1 and form the apoptosome that activates caspase-9, a caspase that cleaves and activates caspase-3.	bind
35580	2	8571	7	NULL	NULL	0	NULL	Apaf-1	NULL		is a type of	NULL				adaptor molecule	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_6_2229_s_244	12466137	63  The cytochrome c is known to bind with the adaptor molecule Apaf-1 and form the apoptosome that activates caspase-9, a caspase that cleaves and activates caspase-3.	bind
35581	3	8571	7	NULL	NULL	0	NULL	statement 1	NULL		forms	NULL				apoptosome	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_6_2229_s_244	12466137	63  The cytochrome c is known to bind with the adaptor molecule Apaf-1 and form the apoptosome that activates caspase-9, a caspase that cleaves and activates caspase-3.	bind
35582	4	8571	7	NULL	NULL	0	NULL	apoptosome	NULL		activates	NULL				caspase-9	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_6_2229_s_244	12466137	63  The cytochrome c is known to bind with the adaptor molecule Apaf-1 and form the apoptosome that activates caspase-9, a caspase that cleaves and activates caspase-3.	bind
35583	5	8571	7	NULL	NULL	0	NULL	 caspase-9	NULL		cleaves	NULL				caspase-3	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_6_2229_s_244	12466137	63  The cytochrome c is known to bind with the adaptor molecule Apaf-1 and form the apoptosome that activates caspase-9, a caspase that cleaves and activates caspase-3.	bind
35584	6	8571	7	NULL	NULL	0	NULL	caspase-9	NULL		activates	NULL				caspase-3	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_6_2229_s_244	12466137	63  The cytochrome c is known to bind with the adaptor molecule Apaf-1 and form the apoptosome that activates caspase-9, a caspase that cleaves and activates caspase-3.	bind
34191	1	8572	5	13	NULL	NULL	NULL	gp120	GP		is a type of					viral proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_5_1599_s_327	10550317	63 Binding of viral proteins (gp120) and SDF-1 to CXCR4 expressed on neurons could be a pathway for the neuronal apoptosis, suggesting an additional mechanism for neurodegeneration developed in HAD and HIVE.	bind
34193	2	8572	5	13	NULL	NULL	NULL	CXCR4	GP		is expressed on					neurons	Cell				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_5_1599_s_327	10550317	63 Binding of viral proteins (gp120) and SDF-1 to CXCR4 expressed on neurons could be a pathway for the neuronal apoptosis, suggesting an additional mechanism for neurodegeneration developed in HAD and HIVE.	bind
34195	3	8572	5	13	NULL	NULL	NULL	gp120	GP		bind					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_5_1599_s_327	10550317	63 Binding of viral proteins (gp120) and SDF-1 to CXCR4 expressed on neurons could be a pathway for the neuronal apoptosis, suggesting an additional mechanism for neurodegeneration developed in HAD and HIVE.	bind
34196	4	8572	5	13	NULL	NULL	NULL	SDF-1	GP		bind					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_5_1599_s_327	10550317	63 Binding of viral proteins (gp120) and SDF-1 to CXCR4 expressed on neurons could be a pathway for the neuronal apoptosis, suggesting an additional mechanism for neurodegeneration developed in HAD and HIVE.	bind
34200	5	8572	5	13	NULL	NULL	NULL	statement 3	Process		pathway for		could be			neuronal apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_5_1599_s_327	10550317	63 Binding of viral proteins (gp120) and SDF-1 to CXCR4 expressed on neurons could be a pathway for the neuronal apoptosis, suggesting an additional mechanism for neurodegeneration developed in HAD and HIVE.	bind
34202	6	8572	5	13	NULL	NULL	NULL	statement 4	Process		pathway for		could be			neuronal apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_5_1599_s_327	10550317	63 Binding of viral proteins (gp120) and SDF-1 to CXCR4 expressed on neurons could be a pathway for the neuronal apoptosis, suggesting an additional mechanism for neurodegeneration developed in HAD and HIVE.	bind
35585	6	8572	7	10	NULL	0	NULL	gp120			bind					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_5_1599_s_327	10550317	63 Binding of viral proteins (gp120) and SDF-1 to CXCR4 expressed on neurons could be a pathway for the neuronal apoptosis, suggesting an additional mechanism for neurodegeneration developed in HAD and HIVE.	bind
35586	2	8572	7	NULL	NULL	0	NULL	gp 120	NULL		is a type of	NULL				viral protein	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_5_1599_s_327	10550317	63 Binding of viral proteins (gp120) and SDF-1 to CXCR4 expressed on neurons could be a pathway for the neuronal apoptosis, suggesting an additional mechanism for neurodegeneration developed in HAD and HIVE.	bind
35587	3	8572	7	10	NULL	0	NULL	SDF-1			bind					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_5_1599_s_327	10550317	63 Binding of viral proteins (gp120) and SDF-1 to CXCR4 expressed on neurons could be a pathway for the neuronal apoptosis, suggesting an additional mechanism for neurodegeneration developed in HAD and HIVE.	bind
35588	4	8572	7	NULL	NULL	0	NULL	statement 1	NULL		pathway for	NULL				neuronal apoptosis	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_5_1599_s_327	10550317	63 Binding of viral proteins (gp120) and SDF-1 to CXCR4 expressed on neurons could be a pathway for the neuronal apoptosis, suggesting an additional mechanism for neurodegeneration developed in HAD and HIVE.	bind
35589	5	8572	7	NULL	NULL	0	NULL	statement 2	NULL		pathway for	NULL				neuronal apoptosis	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_5_1599_s_327	10550317	63 Binding of viral proteins (gp120) and SDF-1 to CXCR4 expressed on neurons could be a pathway for the neuronal apoptosis, suggesting an additional mechanism for neurodegeneration developed in HAD and HIVE.	bind
55813	1	8572	7	10	NULL	0	NULL	CXCR4			is expressed in					neurons					NULL		0	NULL	NULL	NULL	gw60_amjpathol_155_5_1599_s_327	10550317	63 Binding of viral proteins (gp120) and SDF-1 to CXCR4 expressed on neurons could be a pathway for the neuronal apoptosis, suggesting an additional mechanism for neurodegeneration developed in HAD and HIVE.	bind
34178	1	8573	5	13	NULL	NULL	NULL	cGKIalpha	GP		bind					MLC phosphatase	GP		myosin-binding subunit		NULL		NULL	NULL	NULL	NULL	gw70_circulation_108_18_2172_s_78	14597579	63 cGKIalpha binds to and phosphorylates the myosin-binding subunit of MLC phosphatase, which could be important for localization of cGKI near the enzyme it regulates.	bind
34180	2	8573	5	13	NULL	NULL	NULL	statement 1	Process		phosphorylates					MLC phosphatase	GP		myosin-binding subunit		NULL		NULL	NULL	NULL	NULL	gw70_circulation_108_18_2172_s_78	14597579	63 cGKIalpha binds to and phosphorylates the myosin-binding subunit of MLC phosphatase, which could be important for localization of cGKI near the enzyme it regulates.	bind
34214	3	8573	5	13	NULL	NULL	NULL	statement 1	Process		is important for					cGKI	GP	localization of 			NULL		NULL	NULL	NULL	NULL	gw70_circulation_108_18_2172_s_78	14597579	63 cGKIalpha binds to and phosphorylates the myosin-binding subunit of MLC phosphatase, which could be important for localization of cGKI near the enzyme it regulates.	bind
34215	4	8573	5	13	NULL	NULL	NULL	statement 1	Process		is important for					cGKI	GP	localization of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_108_18_2172_s_78	14597579	63 cGKIalpha binds to and phosphorylates the myosin-binding subunit of MLC phosphatase, which could be important for localization of cGKI near the enzyme it regulates.	bind
35652	1	8573	7	NULL	NULL	0	NULL	cGKIalpha	NULL		binds to	NULL				MLC phosphatase	NULL		myosin-binding subunit		NULL		0	NULL	NULL	NULL	gw70_circulation_108_18_2172_s_78	14597579	63 cGKIalpha binds to and phosphorylates the myosin-binding subunit of MLC phosphatase, which could be important for localization of cGKI near the enzyme it regulates.	bind
35653	2	8573	7	NULL	NULL	0	NULL	cGKIalpha	NULL		phosphorylates	NULL				MLC phosphatase	NULL		 myosin-binding subunit		NULL		0	NULL	NULL	NULL	gw70_circulation_108_18_2172_s_78	14597579	63 cGKIalpha binds to and phosphorylates the myosin-binding subunit of MLC phosphatase, which could be important for localization of cGKI near the enzyme it regulates.	bind
35654	3	8573	7	NULL	NULL	0	NULL	statement 1	NULL		is important for	NULL				cGKI	NULL	localization of			NULL		0	NULL	NULL	NULL	gw70_circulation_108_18_2172_s_78	14597579	63 cGKIalpha binds to and phosphorylates the myosin-binding subunit of MLC phosphatase, which could be important for localization of cGKI near the enzyme it regulates.	bind
35655	4	8573	7	NULL	NULL	0	NULL	statement 2	NULL		is important for	NULL				cGKI	NULL	localization of			NULL		0	NULL	NULL	NULL	gw70_circulation_108_18_2172_s_78	14597579	63 cGKIalpha binds to and phosphorylates the myosin-binding subunit of MLC phosphatase, which could be important for localization of cGKI near the enzyme it regulates.	bind
34222	1	8574	5	13	NULL	NULL	NULL	p300	GP		bind					myocardin	GP		TAD region		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_7_868_s_219	16614312	64 Myocardin HAT activity was dependent on p300 binding to the TAD region (transcriptional activating domain) of myocardin.	bind
34223	2	8574	5	13	NULL	NULL	NULL	TAD region	GP		is					transcriptional activating domain	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_7_868_s_219	16614312	64 Myocardin HAT activity was dependent on p300 binding to the TAD region (transcriptional activating domain) of myocardin.	bind
46682	3	8574	5	13	NULL	NULL	NULL	Myocardin HAT activity	Process		is dependent on					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_7_868_s_219	16614312	64 Myocardin HAT activity was dependent on p300 binding to the TAD region (transcriptional activating domain) of myocardin.	bind
35656	1	8574	7	NULL	NULL	0	NULL	p300	NULL		bind	NULL				myocardin	NULL		TAD region		NULL		0	NULL	NULL	NULL	gw70_circulationres_98_7_868_s_219	16614312	64 Myocardin HAT activity was dependent on p300 binding to the TAD region (transcriptional activating domain) of myocardin.	bind
35657	2	8574	7	NULL	NULL	0	NULL	TAD	NULL		is	NULL				transcriptional activating domain	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_7_868_s_219	16614312	64 Myocardin HAT activity was dependent on p300 binding to the TAD region (transcriptional activating domain) of myocardin.	bind
35658	3	8574	7	NULL	NULL	0	NULL	Myocardin HAT activity	NULL		depends on	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_7_868_s_219	16614312	64 Myocardin HAT activity was dependent on p300 binding to the TAD region (transcriptional activating domain) of myocardin.	bind
34226	1	8575	5	13	NULL	NULL	NULL	Cu	Chemical		bind					SOD1	GP		Cu binding site		NULL		NULL	NULL	NULL	NULL	gw70_jneurosci_24_36_7945_s_164	15356208	64Cu binding to lower-affinity Cu binding sites on SOD1 would not have survived this procedure, and therefore no conclusion about the total stoichiometry of Cu binding to SOD1 can be made from these results.	bind
35659	1	8575	7	10	NULL	0	NULL	Cu			bind					SOD1			Cu binding site		NULL		NULL	NULL	NULL	NULL	gw70_jneurosci_24_36_7945_s_164	15356208	64Cu binding to lower-affinity Cu binding sites on SOD1 would not have survived this procedure, and therefore no conclusion about the total stoichiometry of Cu binding to SOD1 can be made from these results.	bind
34227	1	8576	5	13	NULL	NULL	NULL	FAK	GP		bind					paxillin	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_5_606_s_86	16543511	65 FAK also binds the adapter protein paxillin and tyrosine phosphorylates it at Y31 and Y118, thereby altering paxillin interactions with the alpha4beta1 integrin and the PKL-PIX-PAK complex at the leading edges of spreading lamellipodia.	bind
34228	2	8576	5	13	NULL	NULL	NULL	paxillin	GP		is a type of					adapter protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_5_606_s_86	16543511	65 FAK also binds the adapter protein paxillin and tyrosine phosphorylates it at Y31 and Y118, thereby altering paxillin interactions with the alpha4beta1 integrin and the PKL-PIX-PAK complex at the leading edges of spreading lamellipodia.	bind
34230	3	8576	5	13	NULL	NULL	NULL	statement 1	Process		phosphorylates					paxillin	GP		Y31;;Y118		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_5_606_s_86	16543511	65 FAK also binds the adapter protein paxillin and tyrosine phosphorylates it at Y31 and Y118, thereby altering paxillin interactions with the alpha4beta1 integrin and the PKL-PIX-PAK complex at the leading edges of spreading lamellipodia.	bind
34231	4	8576	5	13	NULL	NULL	NULL	paxillin	GP		interacts with					alpha4beta1 integrin	GP				NULL	at the leading edges of spreading lamellipodia	NULL	NULL	NULL	NULL	gw70_circulationres_98_5_606_s_86	16543511	65 FAK also binds the adapter protein paxillin and tyrosine phosphorylates it at Y31 and Y118, thereby altering paxillin interactions with the alpha4beta1 integrin and the PKL-PIX-PAK complex at the leading edges of spreading lamellipodia.	bind
34232	5	8576	5	13	NULL	NULL	NULL	paxillin	GP		interacts with					PKL-PIX-PAK complex	GP				NULL	at the leading edges of spreading lamellipodia	NULL	NULL	NULL	NULL	gw70_circulationres_98_5_606_s_86	16543511	65 FAK also binds the adapter protein paxillin and tyrosine phosphorylates it at Y31 and Y118, thereby altering paxillin interactions with the alpha4beta1 integrin and the PKL-PIX-PAK complex at the leading edges of spreading lamellipodia.	bind
34233	6	8576	5	13	NULL	NULL	NULL	statement 3	Process		alters					statement 4	Process				NULL	at the leading edges of spreading lamellipodia	NULL	NULL	NULL	NULL	gw70_circulationres_98_5_606_s_86	16543511	65 FAK also binds the adapter protein paxillin and tyrosine phosphorylates it at Y31 and Y118, thereby altering paxillin interactions with the alpha4beta1 integrin and the PKL-PIX-PAK complex at the leading edges of spreading lamellipodia.	bind
34234	7	8576	5	13	NULL	NULL	NULL	statement 3	Process		alters					statement 5	Process				NULL	at the leading edges of spreading lamellipodia	NULL	NULL	NULL	NULL	gw70_circulationres_98_5_606_s_86	16543511	65 FAK also binds the adapter protein paxillin and tyrosine phosphorylates it at Y31 and Y118, thereby altering paxillin interactions with the alpha4beta1 integrin and the PKL-PIX-PAK complex at the leading edges of spreading lamellipodia.	bind
35660	1	8576	7	NULL	NULL	0	NULL	FAK 	NULL		binds	NULL				paxillin	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_5_606_s_86	16543511	65 FAK also binds the adapter protein paxillin and tyrosine phosphorylates it at Y31 and Y118, thereby altering paxillin interactions with the alpha4beta1 integrin and the PKL-PIX-PAK complex at the leading edges of spreading lamellipodia.	bind
35661	2	8576	7	NULL	NULL	0	NULL	Paxillin	NULL		is a type of	NULL				adapter protein	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_5_606_s_86	16543511	65 FAK also binds the adapter protein paxillin and tyrosine phosphorylates it at Y31 and Y118, thereby altering paxillin interactions with the alpha4beta1 integrin and the PKL-PIX-PAK complex at the leading edges of spreading lamellipodia.	bind
35662	3	8576	7	NULL	NULL	0	NULL	FAK	NULL		phosphorylates	NULL				paxillin	NULL		Y31		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_5_606_s_86	16543511	65 FAK also binds the adapter protein paxillin and tyrosine phosphorylates it at Y31 and Y118, thereby altering paxillin interactions with the alpha4beta1 integrin and the PKL-PIX-PAK complex at the leading edges of spreading lamellipodia.	bind
35663	4	8576	7	NULL	NULL	0	NULL	FAK	NULL		phosphorylates	NULL				paxillin	NULL		Y118		NULL		0	NULL	NULL	NULL	gw70_circulationres_98_5_606_s_86	16543511	65 FAK also binds the adapter protein paxillin and tyrosine phosphorylates it at Y31 and Y118, thereby altering paxillin interactions with the alpha4beta1 integrin and the PKL-PIX-PAK complex at the leading edges of spreading lamellipodia.	bind
35664	5	8576	7	10	NULL	0	NULL	paxillin			interacts with					alpha4beta1 integrin					NULL	at the leading edges of spreading lamellipodia	NULL	NULL	NULL	NULL	gw70_circulationres_98_5_606_s_86	16543511	65 FAK also binds the adapter protein paxillin and tyrosine phosphorylates it at Y31 and Y118, thereby altering paxillin interactions with the alpha4beta1 integrin and the PKL-PIX-PAK complex at the leading edges of spreading lamellipodia.	bind
35665	6	8576	7	10	NULL	0	NULL	statement 3			alters					statement 5					NULL	at the leading edges of spreading lamellipodia	NULL	NULL	NULL	NULL	gw70_circulationres_98_5_606_s_86	16543511	65 FAK also binds the adapter protein paxillin and tyrosine phosphorylates it at Y31 and Y118, thereby altering paxillin interactions with the alpha4beta1 integrin and the PKL-PIX-PAK complex at the leading edges of spreading lamellipodia.	bind
35666	7	8576	7	10	NULL	0	NULL	statement 4			alters					statement 5					NULL	at the leading edges of spreading lamellipodia	NULL	NULL	NULL	NULL	gw70_circulationres_98_5_606_s_86	16543511	65 FAK also binds the adapter protein paxillin and tyrosine phosphorylates it at Y31 and Y118, thereby altering paxillin interactions with the alpha4beta1 integrin and the PKL-PIX-PAK complex at the leading edges of spreading lamellipodia.	bind
35667	9	8576	7	10	NULL	0	NULL	statement 3			alters					statement 8					NULL	at the leading edges of spreading lamellipodia	NULL	NULL	NULL	NULL	gw70_circulationres_98_5_606_s_86	16543511	65 FAK also binds the adapter protein paxillin and tyrosine phosphorylates it at Y31 and Y118, thereby altering paxillin interactions with the alpha4beta1 integrin and the PKL-PIX-PAK complex at the leading edges of spreading lamellipodia.	bind
35668	10	8576	7	10	NULL	0	NULL	statement 4			alters					statement 8					NULL	at the leading edges of spreading lamellipodia	NULL	NULL	NULL	NULL	gw70_circulationres_98_5_606_s_86	16543511	65 FAK also binds the adapter protein paxillin and tyrosine phosphorylates it at Y31 and Y118, thereby altering paxillin interactions with the alpha4beta1 integrin and the PKL-PIX-PAK complex at the leading edges of spreading lamellipodia.	bind
35669	8	8576	7	10	NULL	0	NULL	paxillin			interacts with					PKL-PIX-PAK complex					NULL	at the leading edges of spreading lamellipodia	NULL	NULL	NULL	NULL	gw70_circulationres_98_5_606_s_86	16543511	65 FAK also binds the adapter protein paxillin and tyrosine phosphorylates it at Y31 and Y118, thereby altering paxillin interactions with the alpha4beta1 integrin and the PKL-PIX-PAK complex at the leading edges of spreading lamellipodia.	bind
34235	1	8578	5	13	NULL	NULL	NULL	Caveolin	GP		bind		directly			nNOS	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_8_1023_s_165	15117830	66 Caveolin binds directly to nNOS.	bind
35671	1	8578	7	NULL	NULL	0	NULL	Caveolin	NULL		binds	NULL	directly			nNOS	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_8_1023_s_165	15117830	66 Caveolin binds directly to nNOS.	bind
34236	1	8579	5	13	NULL	NULL	NULL	CIB	GP		is					calcium- and integrin-binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_11_1971_s_111	12947018	66,67  Several proteins are known to interact with the cytoplasmic domains of alphaIIb and beta3, and both the calcium- and integrin-binding protein CIB (which binds alphaIIb) and talin (which binds beta3) have been reported to activate alphaIIbbeta3 in vitro.	bind
34237	2	8579	5	13	NULL	NULL	NULL	CIB	GP		bind					alphaIIb	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_11_1971_s_111	12947018	66,67  Several proteins are known to interact with the cytoplasmic domains of alphaIIb and beta3, and both the calcium- and integrin-binding protein CIB (which binds alphaIIb) and talin (which binds beta3) have been reported to activate alphaIIbbeta3 in vitro.	bind
34238	3	8579	5	13	NULL	NULL	NULL	talin	GP		bind					beta3	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_11_1971_s_111	12947018	66,67  Several proteins are known to interact with the cytoplasmic domains of alphaIIb and beta3, and both the calcium- and integrin-binding protein CIB (which binds alphaIIb) and talin (which binds beta3) have been reported to activate alphaIIbbeta3 in vitro.	bind
34239	4	8579	5	13	NULL	NULL	NULL	statement 2	Process		activates					alphaIIbbeta3	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_11_1971_s_111	12947018	66,67  Several proteins are known to interact with the cytoplasmic domains of alphaIIb and beta3, and both the calcium- and integrin-binding protein CIB (which binds alphaIIb) and talin (which binds beta3) have been reported to activate alphaIIbbeta3 in vitro.	bind
34240	5	8579	5	13	NULL	NULL	NULL	statement 3	Process		activates					alphaIIbbeta3	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_11_1971_s_111	12947018	66,67  Several proteins are known to interact with the cytoplasmic domains of alphaIIb and beta3, and both the calcium- and integrin-binding protein CIB (which binds alphaIIb) and talin (which binds beta3) have been reported to activate alphaIIbbeta3 in vitro.	bind
35672	1	8579	7	NULL	NULL	0	NULL	CIB	NULL		binds	NULL				alphaIIb	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_11_1971_s_111	12947018	66,67  Several proteins are known to interact with the cytoplasmic domains of alphaIIb and beta3, and both the calcium- and integrin-binding protein CIB (which binds alphaIIb) and talin (which binds beta3) have been reported to activate alphaIIbbeta3 in vitro.	bind
35673	2	8579	7	10	NULL	0	NULL	CIB			is					calcium- and integrin-binding protein					NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_11_1971_s_111	12947018	66,67  Several proteins are known to interact with the cytoplasmic domains of alphaIIb and beta3, and both the calcium- and integrin-binding protein CIB (which binds alphaIIb) and talin (which binds beta3) have been reported to activate alphaIIbbeta3 in vitro.	bind
35674	3	8579	7	NULL	NULL	0	NULL	talin	NULL		binds	NULL				beta3	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_11_1971_s_111	12947018	66,67  Several proteins are known to interact with the cytoplasmic domains of alphaIIb and beta3, and both the calcium- and integrin-binding protein CIB (which binds alphaIIb) and talin (which binds beta3) have been reported to activate alphaIIbbeta3 in vitro.	bind
35677	4	8579	7	NULL	NULL	0	NULL	CIB 	NULL		activate	NULL				alphaIIbbeta3	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_11_1971_s_111	12947018	66,67  Several proteins are known to interact with the cytoplasmic domains of alphaIIb and beta3, and both the calcium- and integrin-binding protein CIB (which binds alphaIIb) and talin (which binds beta3) have been reported to activate alphaIIbbeta3 in vitro.	bind
35678	5	8579	7	NULL	NULL	0	NULL	talin 	NULL		activate	NULL				alphaIIbbeta3	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_11_1971_s_111	12947018	66,67  Several proteins are known to interact with the cytoplasmic domains of alphaIIb and beta3, and both the calcium- and integrin-binding protein CIB (which binds alphaIIb) and talin (which binds beta3) have been reported to activate alphaIIbbeta3 in vitro.	bind
34246	1	8580	5	13	NULL	NULL	NULL	Poly(ADP-ribose) polymerase	GP		bind					transcription factor 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_841_s_411	11160908	67       Butler,A. and Ordahl,C. (1999) Poly(ADP-ribose) polymerase binds with transcription factor 1 to MCAT1 elements to regulate muscle-specific transcription.	bind
34247	2	8580	5	13	NULL	NULL	NULL	statement 1	GP		bind									MCAT1 elements	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_841_s_411	11160908	67       Butler,A. and Ordahl,C. (1999) Poly(ADP-ribose) polymerase binds with transcription factor 1 to MCAT1 elements to regulate muscle-specific transcription.	bind
34248	3	8580	5	13	NULL	NULL	NULL	statement 2	GP		regulates					muscle-specific transcription	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_841_s_411	11160908	67       Butler,A. and Ordahl,C. (1999) Poly(ADP-ribose) polymerase binds with transcription factor 1 to MCAT1 elements to regulate muscle-specific transcription.	bind
35680	1	8580	7	NULL	NULL	0	NULL	Poly(ADP-ribose) polymerase	NULL		bind	NULL				transcription factor 1 	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_841_s_411	11160908	67       Butler,A. and Ordahl,C. (1999) Poly(ADP-ribose) polymerase binds with transcription factor 1 to MCAT1 elements to regulate muscle-specific transcription.	bind
35681	2	8580	7	NULL	NULL	0	NULL	Poly(ADP-ribose) polymerase	NULL		bind	NULL					NULL			MCAT1 elements	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_841_s_411	11160908	67       Butler,A. and Ordahl,C. (1999) Poly(ADP-ribose) polymerase binds with transcription factor 1 to MCAT1 elements to regulate muscle-specific transcription.	bind
35682	3	8580	7	NULL	NULL	0	NULL	statement 2	NULL		regulate	NULL				muscle-specific transcription	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_841_s_411	11160908	67       Butler,A. and Ordahl,C. (1999) Poly(ADP-ribose) polymerase binds with transcription factor 1 to MCAT1 elements to regulate muscle-specific transcription.	bind
34249	1	8581	5	13	NULL	NULL	NULL	Retinyl esters	Chemical		stored in					liver	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1765_s_205	9327775	67  Retinyl esters are either stored in the liver or resecreted as unesterified retinol bound to retinol-binding protein.	bind
34250	2	8581	5	13	NULL	NULL	NULL	retinol	Chemical	unesterified	bind					retinol-binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1765_s_205	9327775	67  Retinyl esters are either stored in the liver or resecreted as unesterified retinol bound to retinol-binding protein.	bind
34251	3	8581	5	13	NULL	NULL	NULL	Retinyl esters	Chemical		resecreted as					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1765_s_205	9327775	67  Retinyl esters are either stored in the liver or resecreted as unesterified retinol bound to retinol-binding protein.	bind
35683	1	8581	7	NULL	NULL	0	NULL	Retinyl esters	NULL		are stored in the	NULL				liver	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1765_s_205	9327775	67  Retinyl esters are either stored in the liver or resecreted as unesterified retinol bound to retinol-binding protein.	bind
35684	2	8581	7	10	NULL	0	NULL	Retinyl esters	NULL		resecreted as	NULL				retinol 	NULL	unesterified 			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1765_s_205	9327775	67  Retinyl esters are either stored in the liver or resecreted as unesterified retinol bound to retinol-binding protein.	bind
35685	3	8581	7	NULL	NULL	0	NULL	statement 2	NULL		binds	NULL				 retinol-binding protein	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_9_1765_s_205	9327775	67  Retinyl esters are either stored in the liver or resecreted as unesterified retinol bound to retinol-binding protein.	bind
36363	1	8582	5	13	NULL	NULL	NULL	SV40 T antigen	GP		bind					pocket protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_4_319_s_228	10455060	67 68 69 70  Consistent with the interpretation that a second region of E1A may be required in addition, it is noteworthy that pocket protein binding by SV40 T antigen did not induce S phase in the presence of dominant-negative Cdk2.	bind
36364	2	8582	5	13	NULL	NULL	NULL	statement 1	Process		does not induce					S phase	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_4_319_s_228	10455060	67 68 69 70  Consistent with the interpretation that a second region of E1A may be required in addition, it is noteworthy that pocket protein binding by SV40 T antigen did not induce S phase in the presence of dominant-negative Cdk2.	bind
36365	3	8582	5	13	NULL	NULL	NULL	statement 2	Process		in the presence of					dominant-negative Cdk2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_4_319_s_228	10455060	67 68 69 70  Consistent with the interpretation that a second region of E1A may be required in addition, it is noteworthy that pocket protein binding by SV40 T antigen did not induce S phase in the presence of dominant-negative Cdk2.	bind
35686	1	8582	7	NULL	NULL	0	NULL	SV40 T antigen	NULL		bind	NULL				pocket protein	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_85_4_319_s_228	10455060	67 68 69 70  Consistent with the interpretation that a second region of E1A may be required in addition, it is noteworthy that pocket protein binding by SV40 T antigen did not induce S phase in the presence of dominant-negative Cdk2.	bind
35687	2	8582	7	NULL	NULL	0	NULL	statement 1	NULL		does not induce	NULL				S phase	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_85_4_319_s_228	10455060	67 68 69 70  Consistent with the interpretation that a second region of E1A may be required in addition, it is noteworthy that pocket protein binding by SV40 T antigen did not induce S phase in the presence of dominant-negative Cdk2.	bind
35688	3	8582	7	NULL	NULL	0	NULL	statement 2	NULL		in the presence of 	NULL				dominant-negative Cdk2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_85_4_319_s_228	10455060	67 68 69 70  Consistent with the interpretation that a second region of E1A may be required in addition, it is noteworthy that pocket protein binding by SV40 T antigen did not induce S phase in the presence of dominant-negative Cdk2.	bind
36366	1	8583	5	13	NULL	NULL	NULL	TFPI	GP		bind					smooth muscle cells	Cell	human			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_4_539_s_158	11950688	67, 68 A synthetic peptide with C-terminal Lys254-Met276 inhibited the binding of TFPI with human smooth muscle cells.	bind
36367	2	8583	5	13	NULL	NULL	NULL	synthetic peptide	GP		inhibit			C-terminal Lys254-Met276		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_4_539_s_158	11950688	67, 68 A synthetic peptide with C-terminal Lys254-Met276 inhibited the binding of TFPI with human smooth muscle cells.	bind
35689	1	8583	7	NULL	NULL	0	NULL	TFPI	NULL		bind	NULL				smooth muscle cells	NULL	human			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_4_539_s_158	11950688	67, 68 A synthetic peptide with C-terminal Lys254-Met276 inhibited the binding of TFPI with human smooth muscle cells.	bind
35690	2	8583	7	NULL	NULL	0	NULL	synthetic peptide	NULL		inhibits	NULL		C-terminal Lys254-Met276		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_4_539_s_158	11950688	67, 68 A synthetic peptide with C-terminal Lys254-Met276 inhibited the binding of TFPI with human smooth muscle cells.	bind
36368	1	8585	5	13	NULL	NULL	NULL	6Ckine	GP		bind					CXCR3	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_14_8205_s_113	9653165	6Ckine Binds to CXCR3.	bind
35691	1	8585	7	NULL	NULL	0	NULL	6Ckine	NULL		binds to	NULL				CXCR3	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_14_8205_s_113	9653165	6Ckine Binds to CXCR3.	bind
36369	1	8587	5	13	NULL	NULL	NULL	6HisC-r GRP	GP		bind		dose dependently			LPS	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_insectbiochemmolbiol_33_6_579_s_285	12770576	6HisC-r GRP bound to LPS and LTA in a dose dependent manner that reached  saturation at approximately 10  g/mL ( Fig. 6B).	bind
36370	2	8587	5	13	NULL	NULL	NULL	6HisC-r GRP	GP		bind		dose dependently			LTA	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_insectbiochemmolbiol_33_6_579_s_285	12770576	6HisC-r GRP bound to LPS and LTA in a dose dependent manner that reached  saturation at approximately 10  g/mL ( Fig. 6B).	bind
35695	1	8587	7	NULL	NULL	0	NULL	6HisC-r GRP	NULL		bind	NULL	dose-dependently			LPS	NULL				NULL		0	NULL	NULL	NULL	gw70_insectbiochemmolbiol_33_6_579_s_285	12770576	6HisC-r GRP bound to LPS and LTA in a dose dependent manner that reached  saturation at approximately 10  g/mL ( Fig. 6B).	bind
35696	2	8587	7	NULL	NULL	0	NULL	6HisC-r GRP	NULL		bind	NULL	dose-dependently			LTA	NULL				NULL		0	NULL	NULL	NULL	gw70_insectbiochemmolbiol_33_6_579_s_285	12770576	6HisC-r GRP bound to LPS and LTA in a dose dependent manner that reached  saturation at approximately 10  g/mL ( Fig. 6B).	bind
36371	1	8588	5	13	NULL	NULL	NULL	RNA	NucleicAcid		bind					RNAP	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_101_6_613_s_262	10892648	6S RNA may bind RNAP  in a manner analogous to DNA promoter binding to RNAP.	bind
36372	2	8588	5	13	NULL	NULL	NULL	DNA	NucleicAcid		bind				promoter	RNAP	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_101_6_613_s_262	10892648	6S RNA may bind RNAP  in a manner analogous to DNA promoter binding to RNAP.	bind
36373	3	8588	5	13	NULL	NULL	NULL	statement 1	Process		analogous to		may be			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_101_6_613_s_262	10892648	6S RNA may bind RNAP  in a manner analogous to DNA promoter binding to RNAP.	bind
35697	1	8588	7	NULL	NULL	0	NULL	6S RNA	NULL		bind	NULL	may			RNAP	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_101_6_613_s_262	10892648	6S RNA may bind RNAP  in a manner analogous to DNA promoter binding to RNAP.	bind
35698	2	8588	7	NULL	NULL	0	NULL	RNAP	NULL		bind	NULL				DNA	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_cell_101_6_613_s_262	10892648	6S RNA may bind RNAP  in a manner analogous to DNA promoter binding to RNAP.	bind
35699	3	8588	7	NULL	NULL	0	NULL	statement 1	NULL		is similar to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_101_6_613_s_262	10892648	6S RNA may bind RNAP  in a manner analogous to DNA promoter binding to RNAP.	bind
36374	1	8591	5	13	NULL	NULL	NULL	Vsr	GP		bind					DNA	NucleicAcid	heteroduplex 			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_18_3775_s_265	11557809	7       Drotschmann,K., Aronshtam,A., Fritz,H.J. and Marinus,M.G. (1998) The  Escherichia coli MutL protein stimulates binding of Vsr and MutS to heteroduplex DNA.	bind
36375	2	8591	5	13	NULL	NULL	NULL	MutS	GP		bind					DNA	NucleicAcid	heteroduplex			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_18_3775_s_265	11557809	7       Drotschmann,K., Aronshtam,A., Fritz,H.J. and Marinus,M.G. (1998) The  Escherichia coli MutL protein stimulates binding of Vsr and MutS to heteroduplex DNA.	bind
36376	3	8591	5	13	NULL	NULL	NULL	MutL protein	GP	Escherichia coli	stimulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_18_3775_s_265	11557809	7       Drotschmann,K., Aronshtam,A., Fritz,H.J. and Marinus,M.G. (1998) The  Escherichia coli MutL protein stimulates binding of Vsr and MutS to heteroduplex DNA.	bind
36377	4	8591	5	13	NULL	NULL	NULL	MutL protein	GP	Escherichia coli	stimulate					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_18_3775_s_265	11557809	7       Drotschmann,K., Aronshtam,A., Fritz,H.J. and Marinus,M.G. (1998) The  Escherichia coli MutL protein stimulates binding of Vsr and MutS to heteroduplex DNA.	bind
35700	1	8591	7	10	NULL	0	NULL	Vsr 			bind					DNA		heteroduplex			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_18_3775_s_265	11557809	7       Drotschmann,K., Aronshtam,A., Fritz,H.J. and Marinus,M.G. (1998) The  Escherichia coli MutL protein stimulates binding of Vsr and MutS to heteroduplex DNA.	bind
35701	2	8591	7	10	NULL	0	NULL	MutS			bind					DNA		heteroduplex 			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_18_3775_s_265	11557809	7       Drotschmann,K., Aronshtam,A., Fritz,H.J. and Marinus,M.G. (1998) The  Escherichia coli MutL protein stimulates binding of Vsr and MutS to heteroduplex DNA.	bind
35702	3	8591	7	NULL	NULL	0	NULL	MutL protein	NULL	Escherichia coli	stimulates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_18_3775_s_265	11557809	7       Drotschmann,K., Aronshtam,A., Fritz,H.J. and Marinus,M.G. (1998) The  Escherichia coli MutL protein stimulates binding of Vsr and MutS to heteroduplex DNA.	bind
35703	4	8591	7	NULL	NULL	0	NULL	MutL protein	NULL	Escherichia coli	stimulates	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_18_3775_s_265	11557809	7       Drotschmann,K., Aronshtam,A., Fritz,H.J. and Marinus,M.G. (1998) The  Escherichia coli MutL protein stimulates binding of Vsr and MutS to heteroduplex DNA.	bind
36378	1	8592	5	13	NULL	NULL	NULL	Arc	GP		is a type of					repressor	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2471_s_232	11410653	7       Knight,K.L. and Sauer,R.T. (1989) DNA binding specificity of the Arc and Mnt repressors is determined by a short region of N-terminal residues.	bind
36379	2	8592	5	13	NULL	NULL	NULL	Mnt	GP		is a type of					repressor	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2471_s_232	11410653	7       Knight,K.L. and Sauer,R.T. (1989) DNA binding specificity of the Arc and Mnt repressors is determined by a short region of N-terminal residues.	bind
36380	3	8592	5	13	NULL	NULL	NULL	Arc	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2471_s_232	11410653	7       Knight,K.L. and Sauer,R.T. (1989) DNA binding specificity of the Arc and Mnt repressors is determined by a short region of N-terminal residues.	bind
36381	4	8592	5	13	NULL	NULL	NULL	Mnt	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2471_s_232	11410653	7       Knight,K.L. and Sauer,R.T. (1989) DNA binding specificity of the Arc and Mnt repressors is determined by a short region of N-terminal residues.	bind
35704	1	8592	7	10	NULL	0	NULL	Arc	NULL		bind	NULL				DNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2471_s_232	11410653	7       Knight,K.L. and Sauer,R.T. (1989) DNA binding specificity of the Arc and Mnt repressors is determined by a short region of N-terminal residues.	bind
35705	4	8592	7	10	NULL	0	NULL	Mnt			bind					DNA					NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2471_s_232	11410653	7       Knight,K.L. and Sauer,R.T. (1989) DNA binding specificity of the Arc and Mnt repressors is determined by a short region of N-terminal residues.	bind
46683	3	8592	7	10	NULL	0	NULL	Arc	NULL		is a type of 	NULL				repressor	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2471_s_232	11410653	7       Knight,K.L. and Sauer,R.T. (1989) DNA binding specificity of the Arc and Mnt repressors is determined by a short region of N-terminal residues.	bind
46684	2	8592	7	10	NULL	0	NULL	Mnt	NULL		is a type of 	NULL				repressor	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2471_s_232	11410653	7       Knight,K.L. and Sauer,R.T. (1989) DNA binding specificity of the Arc and Mnt repressors is determined by a short region of N-terminal residues.	bind
36382	1	8593	5	13	NULL	NULL	NULL	TFB homolog	GP	S.shibatae	bind		sequence specific			DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_3_701_s_312	11809882	7       Qureshi,S.A. and Jackson,S.P. (1998) Sequence-specific DNA binding by the  S.shibatae TFB homolog, TFB, and its effect on promoter strength.	bind
36383	2	8593	5	13	NULL	NULL	NULL	TFB	GP		bind		sequence specifically			DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_3_701_s_312	11809882	7       Qureshi,S.A. and Jackson,S.P. (1998) Sequence-specific DNA binding by the  S.shibatae TFB homolog, TFB, and its effect on promoter strength.	bind
35708	1	8593	7	NULL	NULL	0	NULL	TFB homolog	NULL	S.shibatae	bind	NULL	sequence-specific			DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_3_701_s_312	11809882	7       Qureshi,S.A. and Jackson,S.P. (1998) Sequence-specific DNA binding by the  S.shibatae TFB homolog, TFB, and its effect on promoter strength.	bind
35709	2	8593	7	NULL	NULL	0	NULL	TFB	NULL		bind	NULL	sequence-specific			DNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_3_701_s_312	11809882	7       Qureshi,S.A. and Jackson,S.P. (1998) Sequence-specific DNA binding by the  S.shibatae TFB homolog, TFB, and its effect on promoter strength.	bind
36384	1	8594	5	13	NULL	NULL	NULL	Hrp1p	GP		bind									efficiency element	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3377_s_224	11504875	7       Valentini,S.R., Weiss,V.H. and Silver,P.A. (1999) Arginine methylation and binding of Hrp1p to the efficiency element for mRNA 3''-end formation.	bind
36385	2	8594	5	13	NULL	NULL	NULL	statement 1	Process		is required for					mRNA 3''-end	NucleicAcid	formation of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3377_s_224	11504875	7       Valentini,S.R., Weiss,V.H. and Silver,P.A. (1999) Arginine methylation and binding of Hrp1p to the efficiency element for mRNA 3''-end formation.	bind
36386	3	8594	5	13	NULL	NULL	NULL	arginine	AminoAcid	methylation	is required for					mRNA 3''-end	NucleicAcid	formation of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3377_s_224	11504875	7       Valentini,S.R., Weiss,V.H. and Silver,P.A. (1999) Arginine methylation and binding of Hrp1p to the efficiency element for mRNA 3''-end formation.	bind
35710	1	8594	7	10	NULL	0	NULL	Arginine		methylation of	is required for					3'' mRNA		formation of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3377_s_224	11504875	7       Valentini,S.R., Weiss,V.H. and Silver,P.A. (1999) Arginine methylation and binding of Hrp1p to the efficiency element for mRNA 3''-end formation.	bind
35711	2	8594	7	NULL	NULL	0	NULL	 Hrp1p	NULL		bind	NULL					NULL			efficiency element	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3377_s_224	11504875	7       Valentini,S.R., Weiss,V.H. and Silver,P.A. (1999) Arginine methylation and binding of Hrp1p to the efficiency element for mRNA 3''-end formation.	bind
35712	3	8594	7	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				3'' mRNA	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_16_3377_s_224	11504875	7       Valentini,S.R., Weiss,V.H. and Silver,P.A. (1999) Arginine methylation and binding of Hrp1p to the efficiency element for mRNA 3''-end formation.	bind
37635	1	8595	5	13	NULL	NULL	NULL	Pg/Pm	GP		interact with			lysine binding sites of kringle domains		ligand	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_163_2_517_s_18	12875972	7  Binding of Pg and Pm to a variety of cell types occurs, and principally involves interactions of the lysine binding sites of kringle domains of Pg/Pm with appropriate ligands.	bind
35715	1	8595	7	10	NULL	0	NULL	Pg/Pm	NULL		bind	NULL		 lysine binding sites of kringle domain		ligand	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_163_2_517_s_18	12875972	7  Binding of Pg and Pm to a variety of cell types occurs, and principally involves interactions of the lysine binding sites of kringle domains of Pg/Pm with appropriate ligands.	bind
36741	1	8596	5	13	NULL	NULL	NULL	tRA	Chemical		upregulates					CRBP-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_7_1118_s_168	11451739	7  CRBP-1 upregulation is a direct transcriptional effect of tRA, mediated through the binding of retinoic acid receptor (RAR)-alpha to the CRBP-1 promoter.	bind
36742	2	8596	5	13	NULL	NULL	NULL	RAR	GP		is					retinoic acid receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_7_1118_s_168	11451739	7  CRBP-1 upregulation is a direct transcriptional effect of tRA, mediated through the binding of retinoic acid receptor (RAR)-alpha to the CRBP-1 promoter.	bind
36743	3	8596	5	13	NULL	NULL	NULL	(RAR)-alpha	GP		bind					CRBP-1 promoter	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_7_1118_s_168	11451739	7  CRBP-1 upregulation is a direct transcriptional effect of tRA, mediated through the binding of retinoic acid receptor (RAR)-alpha to the CRBP-1 promoter.	bind
36744	4	8596	5	13	NULL	NULL	NULL	statement 3	Process		mediate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_7_1118_s_168	11451739	7  CRBP-1 upregulation is a direct transcriptional effect of tRA, mediated through the binding of retinoic acid receptor (RAR)-alpha to the CRBP-1 promoter.	bind
35717	1	8596	7	NULL	NULL	0	NULL	RAR-alpha	NULL		bind	NULL				CRBP-1	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_7_1118_s_168	11451739	7  CRBP-1 upregulation is a direct transcriptional effect of tRA, mediated through the binding of retinoic acid receptor (RAR)-alpha to the CRBP-1 promoter.	bind
35718	2	8596	7	NULL	NULL	0	NULL	tRA	NULL		upregulates	NULL				CRBP-1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_7_1118_s_168	11451739	7  CRBP-1 upregulation is a direct transcriptional effect of tRA, mediated through the binding of retinoic acid receptor (RAR)-alpha to the CRBP-1 promoter.	bind
35719	3	8596	7	NULL	NULL	0	NULL	statement 2	NULL		transcriptional effect	NULL	direct			tRA	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_7_1118_s_168	11451739	7  CRBP-1 upregulation is a direct transcriptional effect of tRA, mediated through the binding of retinoic acid receptor (RAR)-alpha to the CRBP-1 promoter.	bind
35720	4	8596	7	NULL	NULL	0	NULL	statement 1	NULL		mediates	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_7_1118_s_168	11451739	7  CRBP-1 upregulation is a direct transcriptional effect of tRA, mediated through the binding of retinoic acid receptor (RAR)-alpha to the CRBP-1 promoter.	bind
36738	1	8598	5	13	NULL	NULL	NULL	mucin-like proteins	GP	glycosylated	is expressed by					high endothelial venules	Cell				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_amjpathol_161_5_1607_s_16	12414509	7  In vitro, L-selectin binds to several glycosylated mucin-like proteins expressed by high endothelial venules.	bind
36739	2	8598	5	13	NULL	NULL	NULL	L-selectin	GP		bind					statement 1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_amjpathol_161_5_1607_s_16	12414509	7  In vitro, L-selectin binds to several glycosylated mucin-like proteins expressed by high endothelial venules.	bind
35721	2	8598	7	10	NULL	0	NULL	L-selectin			binds					statement 1					NULL	in vitro	NULL	NULL	NULL	NULL	gw60_amjpathol_161_5_1607_s_16	12414509	7  In vitro, L-selectin binds to several glycosylated mucin-like proteins expressed by high endothelial venules.	bind
35722	1	8598	7	10	NULL	0	NULL	mucin-like proteins		glycosylated	is expressed by					high endothelial venules					NULL	in vitro	NULL	NULL	NULL	NULL	gw60_amjpathol_161_5_1607_s_16	12414509	7  In vitro, L-selectin binds to several glycosylated mucin-like proteins expressed by high endothelial venules.	bind
36745	1	8599	5	13	NULL	NULL	NULL	erbB1	GP		bind		specifically			EGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_18	10381889	7  Ligands that specifically bind to the erbB1, including EGF and several EGF-like gene products, do not directly interact with erbB2 or erbB3, although several recent reports have documented binding of heparin-binding EGF, betacellulin, and epiregulin to erbB4.	bind
36746	2	8599	5	13	NULL	NULL	NULL	erbB1	GP		bind		specifically			EGF-like gene products	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_18	10381889	7  Ligands that specifically bind to the erbB1, including EGF and several EGF-like gene products, do not directly interact with erbB2 or erbB3, although several recent reports have documented binding of heparin-binding EGF, betacellulin, and epiregulin to erbB4.	bind
36749	5	8599	5	13	NULL	NULL	NULL	EGF	GP		does not interact		directly			erbB2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_18	10381889	7  Ligands that specifically bind to the erbB1, including EGF and several EGF-like gene products, do not directly interact with erbB2 or erbB3, although several recent reports have documented binding of heparin-binding EGF, betacellulin, and epiregulin to erbB4.	bind
36750	6	8599	5	13	NULL	NULL	NULL	EGF	GP		does not interact		directly			erbB3	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_18	10381889	7  Ligands that specifically bind to the erbB1, including EGF and several EGF-like gene products, do not directly interact with erbB2 or erbB3, although several recent reports have documented binding of heparin-binding EGF, betacellulin, and epiregulin to erbB4.	bind
36751	7	8599	5	13	NULL	NULL	NULL	statement 5	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_18	10381889	7  Ligands that specifically bind to the erbB1, including EGF and several EGF-like gene products, do not directly interact with erbB2 or erbB3, although several recent reports have documented binding of heparin-binding EGF, betacellulin, and epiregulin to erbB4.	bind
36752	8	8599	5	13	NULL	NULL	NULL	EGF-like gene products	GP		does not interact		directly			erbB2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_18	10381889	7  Ligands that specifically bind to the erbB1, including EGF and several EGF-like gene products, do not directly interact with erbB2 or erbB3, although several recent reports have documented binding of heparin-binding EGF, betacellulin, and epiregulin to erbB4.	bind
36753	9	8599	5	13	NULL	NULL	NULL	EGF-like gene products	GP		does not interact		directly			erbB3	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_18	10381889	7  Ligands that specifically bind to the erbB1, including EGF and several EGF-like gene products, do not directly interact with erbB2 or erbB3, although several recent reports have documented binding of heparin-binding EGF, betacellulin, and epiregulin to erbB4.	bind
36754	10	8599	5	13	NULL	NULL	NULL	statement 8	Process		is an alternative to					statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_18	10381889	7  Ligands that specifically bind to the erbB1, including EGF and several EGF-like gene products, do not directly interact with erbB2 or erbB3, although several recent reports have documented binding of heparin-binding EGF, betacellulin, and epiregulin to erbB4.	bind
36755	11	8599	5	13	NULL	NULL	NULL	EGF	GP		bind					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_18	10381889	7  Ligands that specifically bind to the erbB1, including EGF and several EGF-like gene products, do not directly interact with erbB2 or erbB3, although several recent reports have documented binding of heparin-binding EGF, betacellulin, and epiregulin to erbB4.	bind
36756	12	8599	5	NULL	NULL	0	NULL	statement 11	NULL		bind	NULL				erbB4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_18	10381889	7  Ligands that specifically bind to the erbB1, including EGF and several EGF-like gene products, do not directly interact with erbB2 or erbB3, although several recent reports have documented binding of heparin-binding EGF, betacellulin, and epiregulin to erbB4.	bind
36757	3	8599	5	13	NULL	NULL	NULL	betacellulin	GP		bind					erbB4	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_18	10381889	7  Ligands that specifically bind to the erbB1, including EGF and several EGF-like gene products, do not directly interact with erbB2 or erbB3, although several recent reports have documented binding of heparin-binding EGF, betacellulin, and epiregulin to erbB4.	bind
36758	4	8599	5	13	NULL	NULL	NULL	epiregulin	GP		bind					erbB4	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_18	10381889	7  Ligands that specifically bind to the erbB1, including EGF and several EGF-like gene products, do not directly interact with erbB2 or erbB3, although several recent reports have documented binding of heparin-binding EGF, betacellulin, and epiregulin to erbB4.	bind
35723	1	8599	7	NULL	NULL	0	NULL	EGF	NULL		bind	NULL	specifically			erbB1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_18	10381889	7  Ligands that specifically bind to the erbB1, including EGF and several EGF-like gene products, do not directly interact with erbB2 or erbB3, although several recent reports have documented binding of heparin-binding EGF, betacellulin, and epiregulin to erbB4.	bind
35724	2	8599	7	NULL	NULL	0	NULL	EGF-like gene products	NULL		bind	NULL	specifically			erbB1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_18	10381889	7  Ligands that specifically bind to the erbB1, including EGF and several EGF-like gene products, do not directly interact with erbB2 or erbB3, although several recent reports have documented binding of heparin-binding EGF, betacellulin, and epiregulin to erbB4.	bind
35725	3	8599	7	NULL	NULL	0	NULL	EGF	NULL		does not interact with	NULL	directly			erbB2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_18	10381889	7  Ligands that specifically bind to the erbB1, including EGF and several EGF-like gene products, do not directly interact with erbB2 or erbB3, although several recent reports have documented binding of heparin-binding EGF, betacellulin, and epiregulin to erbB4.	bind
35726	4	8599	7	NULL	NULL	0	NULL	EGF	NULL		does not interact with	NULL	directly			erbB3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_18	10381889	7  Ligands that specifically bind to the erbB1, including EGF and several EGF-like gene products, do not directly interact with erbB2 or erbB3, although several recent reports have documented binding of heparin-binding EGF, betacellulin, and epiregulin to erbB4.	bind
35727	5	8599	7	NULL	NULL	0	NULL	EGF-like gene products	NULL		does not interact with	NULL	directly			erbB2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_18	10381889	7  Ligands that specifically bind to the erbB1, including EGF and several EGF-like gene products, do not directly interact with erbB2 or erbB3, although several recent reports have documented binding of heparin-binding EGF, betacellulin, and epiregulin to erbB4.	bind
35728	6	8599	7	NULL	NULL	0	NULL	EGF-like gene products	NULL		does not interact with	NULL	directly			erbB3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_18	10381889	7  Ligands that specifically bind to the erbB1, including EGF and several EGF-like gene products, do not directly interact with erbB2 or erbB3, although several recent reports have documented binding of heparin-binding EGF, betacellulin, and epiregulin to erbB4.	bind
35729	7	8599	7	NULL	NULL	0	NULL	heparin	NULL		bind	NULL				EGF	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_18	10381889	7  Ligands that specifically bind to the erbB1, including EGF and several EGF-like gene products, do not directly interact with erbB2 or erbB3, although several recent reports have documented binding of heparin-binding EGF, betacellulin, and epiregulin to erbB4.	bind
35730	8	8599	7	10	NULL	0	NULL	betacellulin			bind					erbB4					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_18	10381889	7  Ligands that specifically bind to the erbB1, including EGF and several EGF-like gene products, do not directly interact with erbB2 or erbB3, although several recent reports have documented binding of heparin-binding EGF, betacellulin, and epiregulin to erbB4.	bind
35731	9	8599	7	NULL	NULL	0	NULL	epiregulin	NULL		bind	NULL				erbB4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_18	10381889	7  Ligands that specifically bind to the erbB1, including EGF and several EGF-like gene products, do not directly interact with erbB2 or erbB3, although several recent reports have documented binding of heparin-binding EGF, betacellulin, and epiregulin to erbB4.	bind
56474	10	8599	7	10	NULL	0	NULL	statement 3			is an alternative to					statement 4					NULL		0	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_18	10381889	7  Ligands that specifically bind to the erbB1, including EGF and several EGF-like gene products, do not directly interact with erbB2 or erbB3, although several recent reports have documented binding of heparin-binding EGF, betacellulin, and epiregulin to erbB4.	bind
56475	11	8599	7	10	NULL	0	NULL	statement 5			is an alternative to					statement 6					NULL		0	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_18	10381889	7  Ligands that specifically bind to the erbB1, including EGF and several EGF-like gene products, do not directly interact with erbB2 or erbB3, although several recent reports have documented binding of heparin-binding EGF, betacellulin, and epiregulin to erbB4.	bind
56476	12	8599	7	10	NULL	0	NULL	statement 7			bind					erbB4					NULL		0	NULL	NULL	NULL	gw60_circulationres_84_12_1380_s_18	10381889	7  Ligands that specifically bind to the erbB1, including EGF and several EGF-like gene products, do not directly interact with erbB2 or erbB3, although several recent reports have documented binding of heparin-binding EGF, betacellulin, and epiregulin to erbB4.	bind
36759	1	8600	5	13	NULL	NULL	NULL	thrombin	GP		bind					TM	GP				NULL	endothelial cells	NULL	NULL	NULL	NULL	gw60_circulationres_88_7_681_s_32	11304490	7  On endothelial cells, the inhibition of thrombin binding to TM by a monoclonal antibody 3E2, directed against the fourth EGF-like domain, 8  resulted in an increase of thrombin mitogenic effect.	bind
36760	2	8600	5	13	NULL	NULL	NULL	3E2	GP		is a type of					monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_7_681_s_32	11304490	7  On endothelial cells, the inhibition of thrombin binding to TM by a monoclonal antibody 3E2, directed against the fourth EGF-like domain, 8  resulted in an increase of thrombin mitogenic effect.	bind
36761	3	8600	5	13	NULL	NULL	NULL	3E2	GP		inhibit					statement 1	Process				NULL	endothelial cells	NULL	NULL	NULL	NULL	gw60_circulationres_88_7_681_s_32	11304490	7  On endothelial cells, the inhibition of thrombin binding to TM by a monoclonal antibody 3E2, directed against the fourth EGF-like domain, 8  resulted in an increase of thrombin mitogenic effect.	bind
36762	4	8600	5	13	NULL	NULL	NULL	3E2	GP		is directed against								fourth EGF-like domain		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_7_681_s_32	11304490	7  On endothelial cells, the inhibition of thrombin binding to TM by a monoclonal antibody 3E2, directed against the fourth EGF-like domain, 8  resulted in an increase of thrombin mitogenic effect.	bind
36763	5	8600	5	13	NULL	NULL	NULL	statement 3	Process		increase					thrombin	GP	mitogenic effect of			NULL	endothelial cells	NULL	NULL	NULL	NULL	gw60_circulationres_88_7_681_s_32	11304490	7  On endothelial cells, the inhibition of thrombin binding to TM by a monoclonal antibody 3E2, directed against the fourth EGF-like domain, 8  resulted in an increase of thrombin mitogenic effect.	bind
35732	1	8600	7	NULL	NULL	0	NULL	thrombin	NULL		bind	NULL				TM	NULL				NULL	endothelial cells	0	NULL	NULL	NULL	gw60_circulationres_88_7_681_s_32	11304490	7  On endothelial cells, the inhibition of thrombin binding to TM by a monoclonal antibody 3E2, directed against the fourth EGF-like domain, 8  resulted in an increase of thrombin mitogenic effect.	bind
35733	2	8600	7	10	NULL	0	NULL	3E2			inhibits					statement 1					NULL	endothelial cells	NULL	NULL	NULL	NULL	gw60_circulationres_88_7_681_s_32	11304490	7  On endothelial cells, the inhibition of thrombin binding to TM by a monoclonal antibody 3E2, directed against the fourth EGF-like domain, 8  resulted in an increase of thrombin mitogenic effect.	bind
35734	3	8600	7	10	NULL	0	NULL	3E2			is directed against								 EGF-like domain		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_7_681_s_32	11304490	7  On endothelial cells, the inhibition of thrombin binding to TM by a monoclonal antibody 3E2, directed against the fourth EGF-like domain, 8  resulted in an increase of thrombin mitogenic effect.	bind
35735	4	8600	7	NULL	NULL	0	NULL	statement 2	NULL		increase	NULL				thrombin	NULL	mitogenic effect			NULL		0	NULL	NULL	NULL	gw60_circulationres_88_7_681_s_32	11304490	7  On endothelial cells, the inhibition of thrombin binding to TM by a monoclonal antibody 3E2, directed against the fourth EGF-like domain, 8  resulted in an increase of thrombin mitogenic effect.	bind
55814	5	8600	7	10	NULL	0	NULL	3E2			is a type of					monoclonal antibody					NULL		0	NULL	NULL	NULL	gw60_circulationres_88_7_681_s_32	11304490	7  On endothelial cells, the inhibition of thrombin binding to TM by a monoclonal antibody 3E2, directed against the fourth EGF-like domain, 8  resulted in an increase of thrombin mitogenic effect.	bind
36764	1	8601	5	13	NULL	NULL	NULL	TSP-1	GP		bind					CD36	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_13_1423_s_218	10500044	7  Our data are consistent with the observations of Dawson et al 7  but do not correlate with evidence that the CSVTCG sequence alone, responsible for binding of TSP-1 to CD36, has an effect.	bind
35736	1	8601	7	NULL	NULL	0	NULL	 TSP-1	NULL		bind	NULL				CD36	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_100_13_1423_s_218	10500044	7  Our data are consistent with the observations of Dawson et al 7  but do not correlate with evidence that the CSVTCG sequence alone, responsible for binding of TSP-1 to CD36, has an effect.	bind
37636	1	8602	5	13	NULL	NULL	NULL	shear stress			express					signal transduction regulating gene	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_3_334_s_23	9710127	7  The signal transduction regulating gene expression by shear stress is not exactly defined but appears to include the activation of mitogen-activated protein kinases, 8  9 10  the c-Jun NH2-terminal kinase, 11 12  and modulation of DNA-binding activities of transcription factor activator protein-1 and nuclear factor-kappaB.	bind
37637	2	8602	5	13	NULL	NULL	NULL	statement 1	GP		include		may			mitogen-activated protein kinases	GP	activated			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_3_334_s_23	9710127	7  The signal transduction regulating gene expression by shear stress is not exactly defined but appears to include the activation of mitogen-activated protein kinases, 8  9 10  the c-Jun NH2-terminal kinase, 11 12  and modulation of DNA-binding activities of transcription factor activator protein-1 and nuclear factor-kappaB.	bind
37638	3	8602	5	13	NULL	NULL	NULL	statement 1	GP		include		may			c-Jun NH2-terminal kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_3_334_s_23	9710127	7  The signal transduction regulating gene expression by shear stress is not exactly defined but appears to include the activation of mitogen-activated protein kinases, 8  9 10  the c-Jun NH2-terminal kinase, 11 12  and modulation of DNA-binding activities of transcription factor activator protein-1 and nuclear factor-kappaB.	bind
37639	4	8602	5	13	NULL	NULL	NULL	activator protein-1	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_3_334_s_23	9710127	7  The signal transduction regulating gene expression by shear stress is not exactly defined but appears to include the activation of mitogen-activated protein kinases, 8  9 10  the c-Jun NH2-terminal kinase, 11 12  and modulation of DNA-binding activities of transcription factor activator protein-1 and nuclear factor-kappaB.	bind
37640	5	8602	5	13	NULL	NULL	NULL	nuclear factor-kappaB	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_3_334_s_23	9710127	7  The signal transduction regulating gene expression by shear stress is not exactly defined but appears to include the activation of mitogen-activated protein kinases, 8  9 10  the c-Jun NH2-terminal kinase, 11 12  and modulation of DNA-binding activities of transcription factor activator protein-1 and nuclear factor-kappaB.	bind
37641	6	8602	5	13	NULL	NULL	NULL	nuclear factor-kappaB	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_3_334_s_23	9710127	7  The signal transduction regulating gene expression by shear stress is not exactly defined but appears to include the activation of mitogen-activated protein kinases, 8  9 10  the c-Jun NH2-terminal kinase, 11 12  and modulation of DNA-binding activities of transcription factor activator protein-1 and nuclear factor-kappaB.	bind
37642	7	8602	5	13	NULL	NULL	NULL	activator protein-1	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_3_334_s_23	9710127	7  The signal transduction regulating gene expression by shear stress is not exactly defined but appears to include the activation of mitogen-activated protein kinases, 8  9 10  the c-Jun NH2-terminal kinase, 11 12  and modulation of DNA-binding activities of transcription factor activator protein-1 and nuclear factor-kappaB.	bind
37643	8	8602	5	13	NULL	NULL	NULL	statement 1	Process		include		may			statement 6	Process	modulation of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_3_334_s_23	9710127	7  The signal transduction regulating gene expression by shear stress is not exactly defined but appears to include the activation of mitogen-activated protein kinases, 8  9 10  the c-Jun NH2-terminal kinase, 11 12  and modulation of DNA-binding activities of transcription factor activator protein-1 and nuclear factor-kappaB.	bind
37644	9	8602	5	13	NULL	NULL	NULL	statement 1	Process		include		may			statement 7	Process	modulation of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_3_334_s_23	9710127	7  The signal transduction regulating gene expression by shear stress is not exactly defined but appears to include the activation of mitogen-activated protein kinases, 8  9 10  the c-Jun NH2-terminal kinase, 11 12  and modulation of DNA-binding activities of transcription factor activator protein-1 and nuclear factor-kappaB.	bind
35769	1	8602	7	NULL	NULL	0	NULL	mitogen-activated protein kinases	NULL	activation of	regulates	NULL				gene expression	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_3_334_s_23	9710127	7  The signal transduction regulating gene expression by shear stress is not exactly defined but appears to include the activation of mitogen-activated protein kinases, 8  9 10  the c-Jun NH2-terminal kinase, 11 12  and modulation of DNA-binding activities of transcription factor activator protein-1 and nuclear factor-kappaB.	bind
35770	2	8602	7	NULL	NULL	0	NULL	c-Jun NH2-terminal kinase	NULL		regulates	NULL				gene expression	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_3_334_s_23	9710127	7  The signal transduction regulating gene expression by shear stress is not exactly defined but appears to include the activation of mitogen-activated protein kinases, 8  9 10  the c-Jun NH2-terminal kinase, 11 12  and modulation of DNA-binding activities of transcription factor activator protein-1 and nuclear factor-kappaB.	bind
35771	3	8602	7	NULL	NULL	0	NULL	transcription factor activator protein-1	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_3_334_s_23	9710127	7  The signal transduction regulating gene expression by shear stress is not exactly defined but appears to include the activation of mitogen-activated protein kinases, 8  9 10  the c-Jun NH2-terminal kinase, 11 12  and modulation of DNA-binding activities of transcription factor activator protein-1 and nuclear factor-kappaB.	bind
35772	4	8602	7	NULL	NULL	0	NULL	nuclear factor-kappaB	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_3_334_s_23	9710127	7  The signal transduction regulating gene expression by shear stress is not exactly defined but appears to include the activation of mitogen-activated protein kinases, 8  9 10  the c-Jun NH2-terminal kinase, 11 12  and modulation of DNA-binding activities of transcription factor activator protein-1 and nuclear factor-kappaB.	bind
35773	5	8602	7	NULL	NULL	0	NULL	statement 3	NULL	modulation of	regulates	NULL				gene expression	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_3_334_s_23	9710127	7  The signal transduction regulating gene expression by shear stress is not exactly defined but appears to include the activation of mitogen-activated protein kinases, 8  9 10  the c-Jun NH2-terminal kinase, 11 12  and modulation of DNA-binding activities of transcription factor activator protein-1 and nuclear factor-kappaB.	bind
35774	6	8602	7	NULL	NULL	0	NULL	statement 4	NULL	modulation of	regulates	NULL				gene expression	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_3_334_s_23	9710127	7  The signal transduction regulating gene expression by shear stress is not exactly defined but appears to include the activation of mitogen-activated protein kinases, 8  9 10  the c-Jun NH2-terminal kinase, 11 12  and modulation of DNA-binding activities of transcription factor activator protein-1 and nuclear factor-kappaB.	bind
36765	1	8603	5	13	NULL	NULL	NULL	macrophage	Cell		uptake					CRP - LDL complexes	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_29	15692104	7 - 11     However, macrophage uptake of CRP - LDL complexes might be increased by subsequent binding of CRP to Fcgamma receptors.	bind
36766	2	8603	5	13	NULL	NULL	NULL	CRP	GP		bind					Fcgamma receptors	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_29	15692104	7 - 11     However, macrophage uptake of CRP - LDL complexes might be increased by subsequent binding of CRP to Fcgamma receptors.	bind
36767	3	8603	5	13	NULL	NULL	NULL	statement 2	Process		increase					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_29	15692104	7 - 11     However, macrophage uptake of CRP - LDL complexes might be increased by subsequent binding of CRP to Fcgamma receptors.	bind
35737	1	8603	7	NULL	NULL	0	NULL	CRP	NULL		bind	NULL				Fcgamma receptors	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_29	15692104	7 - 11     However, macrophage uptake of CRP - LDL complexes might be increased by subsequent binding of CRP to Fcgamma receptors.	bind
35738	2	8603	7	10	NULL	0	NULL	macrophage			uptake					 CRP - LDL complexes					NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_29	15692104	7 - 11     However, macrophage uptake of CRP - LDL complexes might be increased by subsequent binding of CRP to Fcgamma receptors.	bind
56152	3	8603	7	10	NULL	0	NULL	statement 1			increase					statement 2					NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_4_717_s_29	15692104	7 - 11     However, macrophage uptake of CRP - LDL complexes might be increased by subsequent binding of CRP to Fcgamma receptors.	bind
36768	1	8604	5	13	NULL	NULL	NULL	immunoglobulin	GP		neutralize					microbial toxin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_6_1604_s_226	7664447	7 13 14  This rapid effect in such children may be due to the neutralization of a microbial toxin by immunoglobulin, which acts as a superantigen that binds nonspecifically to major histocompatibility class II molecules or to certain viable regions of the T-cell - antigen receptor.	bind
36769	2	8604	5	13	NULL	NULL	NULL	immunoglobulin	GP		act as					superantigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_6_1604_s_226	7664447	7 13 14  This rapid effect in such children may be due to the neutralization of a microbial toxin by immunoglobulin, which acts as a superantigen that binds nonspecifically to major histocompatibility class II molecules or to certain viable regions of the T-cell - antigen receptor.	bind
36770	3	8604	5	13	NULL	NULL	NULL	immunoglobulin	GP		bind		nonspecifically			major histocompatibility class II molecules	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_6_1604_s_226	7664447	7 13 14  This rapid effect in such children may be due to the neutralization of a microbial toxin by immunoglobulin, which acts as a superantigen that binds nonspecifically to major histocompatibility class II molecules or to certain viable regions of the T-cell - antigen receptor.	bind
36771	4	8604	5	13	NULL	NULL	NULL	immunoglobulin	GP		bind		nonspecifically			T-cell - antigen receptor	GP	viable regions of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_6_1604_s_226	7664447	7 13 14  This rapid effect in such children may be due to the neutralization of a microbial toxin by immunoglobulin, which acts as a superantigen that binds nonspecifically to major histocompatibility class II molecules or to certain viable regions of the T-cell - antigen receptor.	bind
35739	1	8604	7	NULL	NULL	0	NULL	immunoglobulin	NULL		neutralizes	NULL				microbial toxin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_6_1604_s_226	7664447	7 13 14  This rapid effect in such children may be due to the neutralization of a microbial toxin by immunoglobulin, which acts as a superantigen that binds nonspecifically to major histocompatibility class II molecules or to certain viable regions of the T-cell - antigen receptor.	bind
35740	2	8604	7	NULL	NULL	0	NULL	immunoglobulin	NULL		acts as a 	NULL				superantigen	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_92_6_1604_s_226	7664447	7 13 14  This rapid effect in such children may be due to the neutralization of a microbial toxin by immunoglobulin, which acts as a superantigen that binds nonspecifically to major histocompatibility class II molecules or to certain viable regions of the T-cell - antigen receptor.	bind
35741	3	8604	7	NULL	NULL	0	NULL	immunoglobulin	NULL		binds	NULL	nonspecifically			 major histocompatibility class II molecules	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_6_1604_s_226	7664447	7 13 14  This rapid effect in such children may be due to the neutralization of a microbial toxin by immunoglobulin, which acts as a superantigen that binds nonspecifically to major histocompatibility class II molecules or to certain viable regions of the T-cell - antigen receptor.	bind
35742	4	8604	7	10	NULL	0	NULL	immunoglobulin			binds		nonspecifically			T-cell - antigen receptor		viable regions of 			NULL		NULL	NULL	NULL	NULL	gw60_circulation_92_6_1604_s_226	7664447	7 13 14  This rapid effect in such children may be due to the neutralization of a microbial toxin by immunoglobulin, which acts as a superantigen that binds nonspecifically to major histocompatibility class II molecules or to certain viable regions of the T-cell - antigen receptor.	bind
36772	1	8605	5	13	NULL	NULL	NULL	GP IIb/IIa	GP		bind					vWF	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_5_925_s_27	9157957	7 8  GP IIb/IIa binds to vWF after activation, leading to platelet spreading and aggregation at sites of injury.	bind
36773	2	8605	5	13	NULL	NULL	NULL	statement 1	Process		occurs after					activation	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_5_925_s_27	9157957	7 8  GP IIb/IIa binds to vWF after activation, leading to platelet spreading and aggregation at sites of injury.	bind
36774	3	8605	5	13	NULL	NULL	NULL	statement 1	Process		leads to					platelet spreading	Process				NULL	sites of injury	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_5_925_s_27	9157957	7 8  GP IIb/IIa binds to vWF after activation, leading to platelet spreading and aggregation at sites of injury.	bind
36775	4	8605	5	13	NULL	NULL	NULL	statement 1	Process		leads to					platelet aggregation	Process				NULL	sites of injury	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_5_925_s_27	9157957	7 8  GP IIb/IIa binds to vWF after activation, leading to platelet spreading and aggregation at sites of injury.	bind
35743	1	8605	7	NULL	NULL	0	NULL	GP IIb/IIa	NULL		binds to	NULL				vWF	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_5_925_s_27	9157957	7 8  GP IIb/IIa binds to vWF after activation, leading to platelet spreading and aggregation at sites of injury.	bind
35744	2	8605	7	NULL	NULL	0	NULL	statement 1	NULL		occurs after	NULL				activation	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_5_925_s_27	9157957	7 8  GP IIb/IIa binds to vWF after activation, leading to platelet spreading and aggregation at sites of injury.	bind
35745	3	8605	7	10	NULL	0	NULL	statement 1	NULL		leads to	NULL				platelet spreading	NULL				NULL	sites of injury	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_5_925_s_27	9157957	7 8  GP IIb/IIa binds to vWF after activation, leading to platelet spreading and aggregation at sites of injury.	bind
35746	4	8605	7	10	NULL	0	NULL	statement 1	NULL		leads to	NULL				aggregation	NULL				NULL	sites of injury	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_5_925_s_27	9157957	7 8  GP IIb/IIa binds to vWF after activation, leading to platelet spreading and aggregation at sites of injury.	bind
36776	1	8606	5	13	NULL	NULL	NULL	ERs	GP		bind					17beta-estradiol	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_15_1792_s_24	10769279	7 8  The 2 ERs have a similar affinity for 17beta-estradiol, and they bind to the same estrogen response elements (EREs).	bind
36777	2	8606	5	13	NULL	NULL	NULL	ERs	GP		bind									EREs	NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_15_1792_s_24	10769279	7 8  The 2 ERs have a similar affinity for 17beta-estradiol, and they bind to the same estrogen response elements (EREs).	bind
36778	3	8606	5	13	NULL	NULL	NULL	EREs	GP		is					estrogen response elements	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_15_1792_s_24	10769279	7 8  The 2 ERs have a similar affinity for 17beta-estradiol, and they bind to the same estrogen response elements (EREs).	bind
35749	1	8606	7	10	NULL	0	NULL	ER	NULL		bind	NULL				17beta-estradiol	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_15_1792_s_24	10769279	7 8  The 2 ERs have a similar affinity for 17beta-estradiol, and they bind to the same estrogen response elements (EREs).	bind
35750	2	8606	7	NULL	NULL	0	NULL	ERs	NULL		bind	NULL					NULL			EREs	NULL		0	NULL	NULL	NULL	gw60_circulation_101_15_1792_s_24	10769279	7 8  The 2 ERs have a similar affinity for 17beta-estradiol, and they bind to the same estrogen response elements (EREs).	bind
35751	3	8606	7	NULL	NULL	0	NULL	EREs	NULL		is	NULL				estrogen response elements	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_101_15_1792_s_24	10769279	7 8  The 2 ERs have a similar affinity for 17beta-estradiol, and they bind to the same estrogen response elements (EREs).	bind
36779	1	8607	5	13	NULL	NULL	NULL	PDGF	GP		is secreted as					PDGF-AA	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_11_1330_s_19	10982551	7 8 9 10  PDGF is secreted as 3 different isoforms: PDGF-AA, -AB, and -BB, and binds to 2 distinct subtype receptors, PDGFR-alpha and -beta, which can form homodimers and heterodimers.	bind
36780	2	8607	5	13	NULL	NULL	NULL	PDGF	GP		is secreted as					PDGF-BB	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_11_1330_s_19	10982551	7 8 9 10  PDGF is secreted as 3 different isoforms: PDGF-AA, -AB, and -BB, and binds to 2 distinct subtype receptors, PDGFR-alpha and -beta, which can form homodimers and heterodimers.	bind
36781	3	8607	5	13	NULL	NULL	NULL	PDGF	GP		is secreted as					PDGF-AB	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_11_1330_s_19	10982551	7 8 9 10  PDGF is secreted as 3 different isoforms: PDGF-AA, -AB, and -BB, and binds to 2 distinct subtype receptors, PDGFR-alpha and -beta, which can form homodimers and heterodimers.	bind
36782	4	8607	5	13	NULL	NULL	NULL	PDGF-AA	GP		bind					PDGFR-alpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_11_1330_s_19	10982551	7 8 9 10  PDGF is secreted as 3 different isoforms: PDGF-AA, -AB, and -BB, and binds to 2 distinct subtype receptors, PDGFR-alpha and -beta, which can form homodimers and heterodimers.	bind
36783	5	8607	5	13	NULL	NULL	NULL	PDGF-AA	GP		bind					PDGFR-beta	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_11_1330_s_19	10982551	7 8 9 10  PDGF is secreted as 3 different isoforms: PDGF-AA, -AB, and -BB, and binds to 2 distinct subtype receptors, PDGFR-alpha and -beta, which can form homodimers and heterodimers.	bind
36784	6	8607	5	13	NULL	NULL	NULL	PDGF-AB	GP		bind					PDGFR-alpha 	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_11_1330_s_19	10982551	7 8 9 10  PDGF is secreted as 3 different isoforms: PDGF-AA, -AB, and -BB, and binds to 2 distinct subtype receptors, PDGFR-alpha and -beta, which can form homodimers and heterodimers.	bind
56468	7	8607	5	13	NULL	NULL	NULL	PDGF-AB	GP		bind					PDGFR-beta	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_11_1330_s_19	10982551	7 8 9 10  PDGF is secreted as 3 different isoforms: PDGF-AA, -AB, and -BB, and binds to 2 distinct subtype receptors, PDGFR-alpha and -beta, which can form homodimers and heterodimers.	bind
56469	8	8607	5	13	NULL	NULL	NULL	PDGF-BB	GP		bind					PDGFR-alpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_11_1330_s_19	10982551	7 8 9 10  PDGF is secreted as 3 different isoforms: PDGF-AA, -AB, and -BB, and binds to 2 distinct subtype receptors, PDGFR-alpha and -beta, which can form homodimers and heterodimers.	bind
56470	9	8607	5	13	NULL	NULL	NULL	PDGF-BB	GP		bind					PDGFR-beta	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_11_1330_s_19	10982551	7 8 9 10  PDGF is secreted as 3 different isoforms: PDGF-AA, -AB, and -BB, and binds to 2 distinct subtype receptors, PDGFR-alpha and -beta, which can form homodimers and heterodimers.	bind
56471	10	8607	5	13	NULL	NULL	NULL	PDGFR-alpha	GP		homodimerize with					PDGFR-alpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_11_1330_s_19	10982551	7 8 9 10  PDGF is secreted as 3 different isoforms: PDGF-AA, -AB, and -BB, and binds to 2 distinct subtype receptors, PDGFR-alpha and -beta, which can form homodimers and heterodimers.	bind
56472	11	8607	5	13	NULL	NULL	NULL	PDGFR-beta	GP		homodimerize with					PDGFR-beta	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_11_1330_s_19	10982551	7 8 9 10  PDGF is secreted as 3 different isoforms: PDGF-AA, -AB, and -BB, and binds to 2 distinct subtype receptors, PDGFR-alpha and -beta, which can form homodimers and heterodimers.	bind
56473	12	8607	5	13	NULL	NULL	NULL	PDGFR-alpha	GP		heterodimerize with					PDGFR-beta	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_11_1330_s_19	10982551	7 8 9 10  PDGF is secreted as 3 different isoforms: PDGF-AA, -AB, and -BB, and binds to 2 distinct subtype receptors, PDGFR-alpha and -beta, which can form homodimers and heterodimers.	bind
35752	1	8607	7	NULL	NULL	0	NULL	PDGF-AA	NULL		binds to	NULL				PDGFR-alpha	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_102_11_1330_s_19	10982551	7 8 9 10  PDGF is secreted as 3 different isoforms: PDGF-AA, -AB, and -BB, and binds to 2 distinct subtype receptors, PDGFR-alpha and -beta, which can form homodimers and heterodimers.	bind
35753	2	8607	7	NULL	NULL	0	NULL	PDGF-AA	NULL		binds to	NULL				PDGFR-beta	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_11_1330_s_19	10982551	7 8 9 10  PDGF is secreted as 3 different isoforms: PDGF-AA, -AB, and -BB, and binds to 2 distinct subtype receptors, PDGFR-alpha and -beta, which can form homodimers and heterodimers.	bind
35754	3	8607	7	NULL	NULL	0	NULL	PDGF-AB	NULL		binds to	NULL				 PDGFR-alpha	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_102_11_1330_s_19	10982551	7 8 9 10  PDGF is secreted as 3 different isoforms: PDGF-AA, -AB, and -BB, and binds to 2 distinct subtype receptors, PDGFR-alpha and -beta, which can form homodimers and heterodimers.	bind
35755	4	8607	7	NULL	NULL	0	NULL	PDGF-AB	NULL		binds to	NULL				PDGFR-beta	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_102_11_1330_s_19	10982551	7 8 9 10  PDGF is secreted as 3 different isoforms: PDGF-AA, -AB, and -BB, and binds to 2 distinct subtype receptors, PDGFR-alpha and -beta, which can form homodimers and heterodimers.	bind
35756	5	8607	7	NULL	NULL	0	NULL	PDGF-BB	NULL		binds to	NULL				PDGFR-alpha	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_102_11_1330_s_19	10982551	7 8 9 10  PDGF is secreted as 3 different isoforms: PDGF-AA, -AB, and -BB, and binds to 2 distinct subtype receptors, PDGFR-alpha and -beta, which can form homodimers and heterodimers.	bind
35757	6	8607	7	NULL	NULL	0	NULL	PDGF-BB	NULL		binds to	NULL				PDGFR-beta	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_102_11_1330_s_19	10982551	7 8 9 10  PDGF is secreted as 3 different isoforms: PDGF-AA, -AB, and -BB, and binds to 2 distinct subtype receptors, PDGFR-alpha and -beta, which can form homodimers and heterodimers.	bind
35758	7	8607	7	10	NULL	0	NULL	PDGFR-alpha			 homodimerize with					PDGFR-alpha					NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_11_1330_s_19	10982551	7 8 9 10  PDGF is secreted as 3 different isoforms: PDGF-AA, -AB, and -BB, and binds to 2 distinct subtype receptors, PDGFR-alpha and -beta, which can form homodimers and heterodimers.	bind
35759	8	8607	7	10	NULL	0	NULL	PDGFR-beta			homodimerize with					PDGFR-beta					NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_11_1330_s_19	10982551	7 8 9 10  PDGF is secreted as 3 different isoforms: PDGF-AA, -AB, and -BB, and binds to 2 distinct subtype receptors, PDGFR-alpha and -beta, which can form homodimers and heterodimers.	bind
35760	9	8607	7	10	NULL	0	NULL	PDGFR-alpha			heterodimerize with					PDGFR-beta					NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_11_1330_s_19	10982551	7 8 9 10  PDGF is secreted as 3 different isoforms: PDGF-AA, -AB, and -BB, and binds to 2 distinct subtype receptors, PDGFR-alpha and -beta, which can form homodimers and heterodimers.	bind
36785	1	8608	5	13	NULL	NULL	NULL	calcineurin	GP	activated	bind					NFAT	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1531_s_28	16675727	7 Activated calcineurin binds and dephosphorylates NFAT, which then translocates to the nucleus to activate cells and induce cytokine expression.	bind
36786	2	8608	5	13	NULL	NULL	NULL	statement 1	GP		dephosphorylates					NFAT	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1531_s_28	16675727	7 Activated calcineurin binds and dephosphorylates NFAT, which then translocates to the nucleus to activate cells and induce cytokine expression.	bind
36787	3	8608	5	13	NULL	NULL	NULL	statement 1	GP		is translocated to					nucleus	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1531_s_28	16675727	7 Activated calcineurin binds and dephosphorylates NFAT, which then translocates to the nucleus to activate cells and induce cytokine expression.	bind
36788	4	8608	5	13	NULL	NULL	NULL	statement 3	GP		activates					cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1531_s_28	16675727	7 Activated calcineurin binds and dephosphorylates NFAT, which then translocates to the nucleus to activate cells and induce cytokine expression.	bind
36789	5	8608	5	13	NULL	NULL	NULL	statement 4	Process		induce					cytokine	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1531_s_28	16675727	7 Activated calcineurin binds and dephosphorylates NFAT, which then translocates to the nucleus to activate cells and induce cytokine expression.	bind
35761	1	8608	7	NULL	NULL	0	NULL	calcineurin	NULL	activated	binds	NULL				NFAT	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1531_s_28	16675727	7 Activated calcineurin binds and dephosphorylates NFAT, which then translocates to the nucleus to activate cells and induce cytokine expression.	bind
35762	2	8608	7	NULL	NULL	0	NULL	statement 1	NULL		dephosphorylates	NULL				NFAT	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1531_s_28	16675727	7 Activated calcineurin binds and dephosphorylates NFAT, which then translocates to the nucleus to activate cells and induce cytokine expression.	bind
35763	3	8608	7	NULL	NULL	0	NULL	NFAT	NULL		translocate to	NULL				nucleus	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1531_s_28	16675727	7 Activated calcineurin binds and dephosphorylates NFAT, which then translocates to the nucleus to activate cells and induce cytokine expression.	bind
35764	4	8608	7	NULL	NULL	0	NULL	statement 3	NULL		activates	NULL				cells	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1531_s_28	16675727	7 Activated calcineurin binds and dephosphorylates NFAT, which then translocates to the nucleus to activate cells and induce cytokine expression.	bind
35765	5	8608	7	NULL	NULL	0	NULL	statement 4	NULL		induce	NULL				cytokine expression	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_7_1531_s_28	16675727	7 Activated calcineurin binds and dephosphorylates NFAT, which then translocates to the nucleus to activate cells and induce cytokine expression.	bind
37645	1	8609	5	13	NULL	NULL	NULL	vancomycin	Chemical		bind					cell wall	CellComponent	pre-existing;; modified			NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_43_6_846_s_23	10404328	7 All of these alterations produce a so-called ``trapping effect'' , whereby increased amounts of vancomycin are bound to the pre-existing modified cell wall, thus reducing the amount of drug that reaches its vital targets --  the lipid II precursors of new cell-wall synthesis which are found in the outer leaflet of the cytoplasmic membrane beneath the pre-existing cell wall.	bind
37646	2	8609	5	13	NULL	NULL	NULL	vancomycin	Chemical		reaches					lipid II precursors	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_43_6_846_s_23	10404328	7 All of these alterations produce a so-called ``trapping effect'' , whereby increased amounts of vancomycin are bound to the pre-existing modified cell wall, thus reducing the amount of drug that reaches its vital targets --  the lipid II precursors of new cell-wall synthesis which are found in the outer leaflet of the cytoplasmic membrane beneath the pre-existing cell wall.	bind
37647	3	8609	5	13	NULL	NULL	NULL	lipid II precursors	Chemical		is a type of					vital drug targets	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_43_6_846_s_23	10404328	7 All of these alterations produce a so-called ``trapping effect'' , whereby increased amounts of vancomycin are bound to the pre-existing modified cell wall, thus reducing the amount of drug that reaches its vital targets --  the lipid II precursors of new cell-wall synthesis which are found in the outer leaflet of the cytoplasmic membrane beneath the pre-existing cell wall.	bind
37648	4	8609	5	13	NULL	NULL	NULL	lipid II precursors	Chemical		is present in					cytoplasmic membrane	CellComponent	outer leaflet of			NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_43_6_846_s_23	10404328	7 All of these alterations produce a so-called ``trapping effect'' , whereby increased amounts of vancomycin are bound to the pre-existing modified cell wall, thus reducing the amount of drug that reaches its vital targets --  the lipid II precursors of new cell-wall synthesis which are found in the outer leaflet of the cytoplasmic membrane beneath the pre-existing cell wall.	bind
37649	5	8609	5	13	NULL	NULL	NULL	statement 1	Process	increased amounts of	reduces					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_43_6_846_s_23	10404328	7 All of these alterations produce a so-called ``trapping effect'' , whereby increased amounts of vancomycin are bound to the pre-existing modified cell wall, thus reducing the amount of drug that reaches its vital targets --  the lipid II precursors of new cell-wall synthesis which are found in the outer leaflet of the cytoplasmic membrane beneath the pre-existing cell wall.	bind
35766	1	8609	7	10	NULL	0	NULL	vancomycin			bind					 cell wall		pre-existing;; modified			NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_43_6_846_s_23	10404328	7 All of these alterations produce a so-called ``trapping effect'' , whereby increased amounts of vancomycin are bound to the pre-existing modified cell wall, thus reducing the amount of drug that reaches its vital targets --  the lipid II precursors of new cell-wall synthesis which are found in the outer leaflet of the cytoplasmic membrane beneath the pre-existing cell wall.	bind
35767	2	8609	7	NULL	NULL	0	NULL	lipid II precursors	NULL		is found in the	NULL				cytoplasmic membrane	NULL	outer leaflet of 			NULL		0	NULL	NULL	NULL	gw60_jantimicrobchemoth_43_6_846_s_23	10404328	7 All of these alterations produce a so-called ``trapping effect'' , whereby increased amounts of vancomycin are bound to the pre-existing modified cell wall, thus reducing the amount of drug that reaches its vital targets --  the lipid II precursors of new cell-wall synthesis which are found in the outer leaflet of the cytoplasmic membrane beneath the pre-existing cell wall.	bind
35768	3	8609	7	10	NULL	0	NULL	vancomycin			reaches					lipid II precursors					NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_43_6_846_s_23	10404328	7 All of these alterations produce a so-called ``trapping effect'' , whereby increased amounts of vancomycin are bound to the pre-existing modified cell wall, thus reducing the amount of drug that reaches its vital targets --  the lipid II precursors of new cell-wall synthesis which are found in the outer leaflet of the cytoplasmic membrane beneath the pre-existing cell wall.	bind
56153	4	8609	7	10	NULL	0	NULL	statement 1		increased amounts of	reduces					statement 2					NULL		0	NULL	NULL	NULL	gw60_jantimicrobchemoth_43_6_846_s_23	10404328	7 All of these alterations produce a so-called ``trapping effect'' , whereby increased amounts of vancomycin are bound to the pre-existing modified cell wall, thus reducing the amount of drug that reaches its vital targets --  the lipid II precursors of new cell-wall synthesis which are found in the outer leaflet of the cytoplasmic membrane beneath the pre-existing cell wall.	bind
56155	5	8609	7	10	NULL	0	NULL	lipid II precursors			is a type of					vital drug targets					NULL		0	NULL	NULL	NULL	gw60_jantimicrobchemoth_43_6_846_s_23	10404328	7 All of these alterations produce a so-called ``trapping effect'' , whereby increased amounts of vancomycin are bound to the pre-existing modified cell wall, thus reducing the amount of drug that reaches its vital targets --  the lipid II precursors of new cell-wall synthesis which are found in the outer leaflet of the cytoplasmic membrane beneath the pre-existing cell wall.	bind
36790	1	8611	5	13	NULL	NULL	NULL	BNP	GP		bind					NPR-A	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_6_836_s_26	16061734	7 BNP binds to the natriuretic peptide receptor-A (NPR-A), which is a membrane-bound receptor located on cardiomyocytes, vascular endothelium, smooth muscle, kidneys, and lungs, resulting in activation of its second messenger, cGMP.	bind
36791	2	8611	5	13	NULL	NULL	NULL	NPR-A	GP		is					natriuretic peptide receptor-A	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_6_836_s_26	16061734	7 BNP binds to the natriuretic peptide receptor-A (NPR-A), which is a membrane-bound receptor located on cardiomyocytes, vascular endothelium, smooth muscle, kidneys, and lungs, resulting in activation of its second messenger, cGMP.	bind
36792	3	8611	5	13	NULL	NULL	NULL	NPR-A	GP		is a type of					membrane-bound receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_6_836_s_26	16061734	7 BNP binds to the natriuretic peptide receptor-A (NPR-A), which is a membrane-bound receptor located on cardiomyocytes, vascular endothelium, smooth muscle, kidneys, and lungs, resulting in activation of its second messenger, cGMP.	bind
36793	4	8611	5	13	NULL	NULL	NULL	NPR-A	GP		is located on					cardiomyocytes	Cell				NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_6_836_s_26	16061734	7 BNP binds to the natriuretic peptide receptor-A (NPR-A), which is a membrane-bound receptor located on cardiomyocytes, vascular endothelium, smooth muscle, kidneys, and lungs, resulting in activation of its second messenger, cGMP.	bind
36795	9	8611	5	13	NULL	NULL	NULL	cGMP	Chemical		is a type of					second messenger	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_6_836_s_26	16061734	7 BNP binds to the natriuretic peptide receptor-A (NPR-A), which is a membrane-bound receptor located on cardiomyocytes, vascular endothelium, smooth muscle, kidneys, and lungs, resulting in activation of its second messenger, cGMP.	bind
36796	5	8611	5	13	NULL	NULL	NULL	NPR-A	GP		is located on					vascular endothelium	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_6_836_s_26	16061734	7 BNP binds to the natriuretic peptide receptor-A (NPR-A), which is a membrane-bound receptor located on cardiomyocytes, vascular endothelium, smooth muscle, kidneys, and lungs, resulting in activation of its second messenger, cGMP.	bind
36798	6	8611	5	13	NULL	NULL	NULL	NPR-A	GP		is located on					smooth muscle	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_6_836_s_26	16061734	7 BNP binds to the natriuretic peptide receptor-A (NPR-A), which is a membrane-bound receptor located on cardiomyocytes, vascular endothelium, smooth muscle, kidneys, and lungs, resulting in activation of its second messenger, cGMP.	bind
36800	7	8611	5	13	NULL	NULL	NULL	NPR-A	GP		is located on					kidneys	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_6_836_s_26	16061734	7 BNP binds to the natriuretic peptide receptor-A (NPR-A), which is a membrane-bound receptor located on cardiomyocytes, vascular endothelium, smooth muscle, kidneys, and lungs, resulting in activation of its second messenger, cGMP.	bind
36801	10	8611	5	13	NULL	NULL	NULL	statement 1	Process		activates					cGMP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_6_836_s_26	16061734	7 BNP binds to the natriuretic peptide receptor-A (NPR-A), which is a membrane-bound receptor located on cardiomyocytes, vascular endothelium, smooth muscle, kidneys, and lungs, resulting in activation of its second messenger, cGMP.	bind
36802	8	8611	5	13	NULL	NULL	NULL	NPR-A	GP		is located on					lungs	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_6_836_s_26	16061734	7 BNP binds to the natriuretic peptide receptor-A (NPR-A), which is a membrane-bound receptor located on cardiomyocytes, vascular endothelium, smooth muscle, kidneys, and lungs, resulting in activation of its second messenger, cGMP.	bind
35918	1	8611	7	NULL	NULL	0	NULL	BNP	NULL		binds to	NULL				NPR-A	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_112_6_836_s_26	16061734	7 BNP binds to the natriuretic peptide receptor-A (NPR-A), which is a membrane-bound receptor located on cardiomyocytes, vascular endothelium, smooth muscle, kidneys, and lungs, resulting in activation of its second messenger, cGMP.	bind
35919	2	8611	7	NULL	NULL	0	NULL	NPR-A	NULL		is	NULL				natriuretic peptide receptor-A	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_112_6_836_s_26	16061734	7 BNP binds to the natriuretic peptide receptor-A (NPR-A), which is a membrane-bound receptor located on cardiomyocytes, vascular endothelium, smooth muscle, kidneys, and lungs, resulting in activation of its second messenger, cGMP.	bind
35920	3	8611	7	NULL	NULL	0	NULL	NPR-A	NULL		is a type of	NULL				membrane-bound receptor	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_112_6_836_s_26	16061734	7 BNP binds to the natriuretic peptide receptor-A (NPR-A), which is a membrane-bound receptor located on cardiomyocytes, vascular endothelium, smooth muscle, kidneys, and lungs, resulting in activation of its second messenger, cGMP.	bind
35921	4	8611	7	NULL	NULL	0	NULL	NPR-A	NULL		is located on 	NULL				cardiomyocytes	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_112_6_836_s_26	16061734	7 BNP binds to the natriuretic peptide receptor-A (NPR-A), which is a membrane-bound receptor located on cardiomyocytes, vascular endothelium, smooth muscle, kidneys, and lungs, resulting in activation of its second messenger, cGMP.	bind
35922	5	8611	7	NULL	NULL	0	NULL	NPR-A	NULL		is located on	NULL				vascular endothelium	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_112_6_836_s_26	16061734	7 BNP binds to the natriuretic peptide receptor-A (NPR-A), which is a membrane-bound receptor located on cardiomyocytes, vascular endothelium, smooth muscle, kidneys, and lungs, resulting in activation of its second messenger, cGMP.	bind
35923	6	8611	7	NULL	NULL	0	NULL	NPR-A	NULL		is located on	NULL				smooth muscle	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_112_6_836_s_26	16061734	7 BNP binds to the natriuretic peptide receptor-A (NPR-A), which is a membrane-bound receptor located on cardiomyocytes, vascular endothelium, smooth muscle, kidneys, and lungs, resulting in activation of its second messenger, cGMP.	bind
35924	7	8611	7	NULL	NULL	0	NULL	NPR-A	NULL		is located on	NULL				kidneys	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_112_6_836_s_26	16061734	7 BNP binds to the natriuretic peptide receptor-A (NPR-A), which is a membrane-bound receptor located on cardiomyocytes, vascular endothelium, smooth muscle, kidneys, and lungs, resulting in activation of its second messenger, cGMP.	bind
35925	8	8611	7	NULL	NULL	0	NULL	NPR-A	NULL		is located on	NULL				lungs	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_112_6_836_s_26	16061734	7 BNP binds to the natriuretic peptide receptor-A (NPR-A), which is a membrane-bound receptor located on cardiomyocytes, vascular endothelium, smooth muscle, kidneys, and lungs, resulting in activation of its second messenger, cGMP.	bind
35926	9	8611	7	NULL	NULL	0	NULL	statement 1	NULL		results in	NULL				cGMP	NULL	activation of			NULL		0	NULL	NULL	NULL	gw70_circulation_112_6_836_s_26	16061734	7 BNP binds to the natriuretic peptide receptor-A (NPR-A), which is a membrane-bound receptor located on cardiomyocytes, vascular endothelium, smooth muscle, kidneys, and lungs, resulting in activation of its second messenger, cGMP.	bind
35927	10	8611	7	NULL	NULL	0	NULL	cGMP	NULL		is a type of	NULL				second messenger	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_112_6_836_s_26	16061734	7 BNP binds to the natriuretic peptide receptor-A (NPR-A), which is a membrane-bound receptor located on cardiomyocytes, vascular endothelium, smooth muscle, kidneys, and lungs, resulting in activation of its second messenger, cGMP.	bind
36803	1	8612	5	13	NULL	NULL	NULL	ES	Chemical		bind					KDR	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_9_1203_s_25	16574906	7 ES was found to bind to the VEGF receptor kinase - inserted domain-containing receptor (KDR), thereby blocking tyrosine phosphorylation and the activation of mitogen-activated protein kinase (MAPK), which leads to an inhibition of VEGF-induced migration and proliferation.	bind
36804	2	8612	5	13	NULL	NULL	NULL	KDR	GP		is					kinase - inserted domain-containing receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_9_1203_s_25	16574906	7 ES was found to bind to the VEGF receptor kinase - inserted domain-containing receptor (KDR), thereby blocking tyrosine phosphorylation and the activation of mitogen-activated protein kinase (MAPK), which leads to an inhibition of VEGF-induced migration and proliferation.	bind
36805	3	8612	5	13	NULL	NULL	NULL	KDR	GP		is a type of					VEGF receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_9_1203_s_25	16574906	7 ES was found to bind to the VEGF receptor kinase - inserted domain-containing receptor (KDR), thereby blocking tyrosine phosphorylation and the activation of mitogen-activated protein kinase (MAPK), which leads to an inhibition of VEGF-induced migration and proliferation.	bind
36806	4	8612	5	13	NULL	NULL	NULL	statement 1	Process		block					MAPK	GP	phosphorylation of	tyrosine		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_9_1203_s_25	16574906	7 ES was found to bind to the VEGF receptor kinase - inserted domain-containing receptor (KDR), thereby blocking tyrosine phosphorylation and the activation of mitogen-activated protein kinase (MAPK), which leads to an inhibition of VEGF-induced migration and proliferation.	bind
36807	5	8612	5	13	NULL	NULL	NULL	statement 1	Process		block					MAPK	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_9_1203_s_25	16574906	7 ES was found to bind to the VEGF receptor kinase - inserted domain-containing receptor (KDR), thereby blocking tyrosine phosphorylation and the activation of mitogen-activated protein kinase (MAPK), which leads to an inhibition of VEGF-induced migration and proliferation.	bind
36808	6	8612	5	13	NULL	NULL	NULL	MAPK	GP		is					mitogen-activated protein kinase	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_9_1203_s_25	16574906	7 ES was found to bind to the VEGF receptor kinase - inserted domain-containing receptor (KDR), thereby blocking tyrosine phosphorylation and the activation of mitogen-activated protein kinase (MAPK), which leads to an inhibition of VEGF-induced migration and proliferation.	bind
36809	7	8612	5	13	NULL	NULL	NULL	VEGF	GP		induce					migration	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_9_1203_s_25	16574906	7 ES was found to bind to the VEGF receptor kinase - inserted domain-containing receptor (KDR), thereby blocking tyrosine phosphorylation and the activation of mitogen-activated protein kinase (MAPK), which leads to an inhibition of VEGF-induced migration and proliferation.	bind
36810	8	8612	5	13	NULL	NULL	NULL	VEGF	GP		induce					proliferation	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_9_1203_s_25	16574906	7 ES was found to bind to the VEGF receptor kinase - inserted domain-containing receptor (KDR), thereby blocking tyrosine phosphorylation and the activation of mitogen-activated protein kinase (MAPK), which leads to an inhibition of VEGF-induced migration and proliferation.	bind
36811	9	8612	5	13	NULL	NULL	NULL	MAPK	GP	activation of	inhibit					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_9_1203_s_25	16574906	7 ES was found to bind to the VEGF receptor kinase - inserted domain-containing receptor (KDR), thereby blocking tyrosine phosphorylation and the activation of mitogen-activated protein kinase (MAPK), which leads to an inhibition of VEGF-induced migration and proliferation.	bind
36812	10	8612	5	13	NULL	NULL	NULL	MAPK	GP	activation of	inhibit					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_9_1203_s_25	16574906	7 ES was found to bind to the VEGF receptor kinase - inserted domain-containing receptor (KDR), thereby blocking tyrosine phosphorylation and the activation of mitogen-activated protein kinase (MAPK), which leads to an inhibition of VEGF-induced migration and proliferation.	bind
35928	1	8612	7	NULL	NULL	0	NULL	ES	NULL		bind	NULL				KDR	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_9_1203_s_25	16574906	7 ES was found to bind to the VEGF receptor kinase - inserted domain-containing receptor (KDR), thereby blocking tyrosine phosphorylation and the activation of mitogen-activated protein kinase (MAPK), which leads to an inhibition of VEGF-induced migration and proliferation.	bind
35929	2	8612	7	10	NULL	0	NULL	statement 1			blocks					MAPK		phosphorylation of	tyrosine		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_9_1203_s_25	16574906	7 ES was found to bind to the VEGF receptor kinase - inserted domain-containing receptor (KDR), thereby blocking tyrosine phosphorylation and the activation of mitogen-activated protein kinase (MAPK), which leads to an inhibition of VEGF-induced migration and proliferation.	bind
35930	3	8612	7	NULL	NULL	0	NULL	statement 1	NULL		blocks	NULL				MAPK	NULL	activation of			NULL		0	NULL	NULL	NULL	gw70_circulationres_98_9_1203_s_25	16574906	7 ES was found to bind to the VEGF receptor kinase - inserted domain-containing receptor (KDR), thereby blocking tyrosine phosphorylation and the activation of mitogen-activated protein kinase (MAPK), which leads to an inhibition of VEGF-induced migration and proliferation.	bind
35931	4	8612	7	NULL	NULL	0	NULL	VEGF	NULL		induce	NULL				migration	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_9_1203_s_25	16574906	7 ES was found to bind to the VEGF receptor kinase - inserted domain-containing receptor (KDR), thereby blocking tyrosine phosphorylation and the activation of mitogen-activated protein kinase (MAPK), which leads to an inhibition of VEGF-induced migration and proliferation.	bind
35932	5	8612	7	NULL	NULL	0	NULL	VEGF	NULL		induce	NULL				proliferation	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_9_1203_s_25	16574906	7 ES was found to bind to the VEGF receptor kinase - inserted domain-containing receptor (KDR), thereby blocking tyrosine phosphorylation and the activation of mitogen-activated protein kinase (MAPK), which leads to an inhibition of VEGF-induced migration and proliferation.	bind
35933	6	8612	7	10	NULL	0	NULL	MAPK		activation of	inhibits					statement 4					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_9_1203_s_25	16574906	7 ES was found to bind to the VEGF receptor kinase - inserted domain-containing receptor (KDR), thereby blocking tyrosine phosphorylation and the activation of mitogen-activated protein kinase (MAPK), which leads to an inhibition of VEGF-induced migration and proliferation.	bind
35934	7	8612	7	10	NULL	0	NULL	MAPK		activation of	inhibits					statement 5					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_9_1203_s_25	16574906	7 ES was found to bind to the VEGF receptor kinase - inserted domain-containing receptor (KDR), thereby blocking tyrosine phosphorylation and the activation of mitogen-activated protein kinase (MAPK), which leads to an inhibition of VEGF-induced migration and proliferation.	bind
35935	8	8612	7	NULL	NULL	0	NULL	KDR	NULL		is	NULL				VEGF receptor kinase - inserted domain-containing receptor	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_9_1203_s_25	16574906	7 ES was found to bind to the VEGF receptor kinase - inserted domain-containing receptor (KDR), thereby blocking tyrosine phosphorylation and the activation of mitogen-activated protein kinase (MAPK), which leads to an inhibition of VEGF-induced migration and proliferation.	bind
56477	9	8612	7	10	NULL	0	NULL	MAPK			is 					mitogen-activated protein kinase					NULL		0	NULL	NULL	NULL	gw70_circulationres_98_9_1203_s_25	16574906	7 ES was found to bind to the VEGF receptor kinase - inserted domain-containing receptor (KDR), thereby blocking tyrosine phosphorylation and the activation of mitogen-activated protein kinase (MAPK), which leads to an inhibition of VEGF-induced migration and proliferation.	bind
56478	10	8612	7	10	NULL	0	NULL	KDR			is a type of					VEGF receptor					NULL		0	NULL	NULL	NULL	gw70_circulationres_98_9_1203_s_25	16574906	7 ES was found to bind to the VEGF receptor kinase - inserted domain-containing receptor (KDR), thereby blocking tyrosine phosphorylation and the activation of mitogen-activated protein kinase (MAPK), which leads to an inhibition of VEGF-induced migration and proliferation.	bind
36813	1	8613	5	13	NULL	NULL	NULL	Trx1	GP	reduced form of	bind					ASK1	GP		N-terminal		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1483_s_39	15117824	7 Interestingly, only the reduced form of Trx1 binds to the N-terminal part of ASK1 and blocks activation of ASK1 by TNF. 7,9  Neither the oxidized form (intramolecular disulfide between C32 and C35) nor the redox-inactive form (the double-mutation at catalytic sites C32 and C35) of Trx1 binds to ASK1.	bind
36814	2	8613	5	13	NULL	NULL	NULL	ASK1	GP		is activated by					TNF	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1483_s_39	15117824	7 Interestingly, only the reduced form of Trx1 binds to the N-terminal part of ASK1 and blocks activation of ASK1 by TNF. 7,9  Neither the oxidized form (intramolecular disulfide between C32 and C35) nor the redox-inactive form (the double-mutation at catalytic sites C32 and C35) of Trx1 binds to ASK1.	bind
36815	3	8613	5	13	NULL	NULL	NULL	statement 1	Process		block					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1483_s_39	15117824	7 Interestingly, only the reduced form of Trx1 binds to the N-terminal part of ASK1 and blocks activation of ASK1 by TNF. 7,9  Neither the oxidized form (intramolecular disulfide between C32 and C35) nor the redox-inactive form (the double-mutation at catalytic sites C32 and C35) of Trx1 binds to ASK1.	bind
36816	4	8613	5	13	NULL	NULL	NULL	Trx1	GP	oxidized form	does not bind					ASK1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1483_s_39	15117824	7 Interestingly, only the reduced form of Trx1 binds to the N-terminal part of ASK1 and blocks activation of ASK1 by TNF. 7,9  Neither the oxidized form (intramolecular disulfide between C32 and C35) nor the redox-inactive form (the double-mutation at catalytic sites C32 and C35) of Trx1 binds to ASK1.	bind
36817	5	8613	5	13	NULL	NULL	NULL	Trx1	GP	redox-inactive form	does not bind					ASK1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1483_s_39	15117824	7 Interestingly, only the reduced form of Trx1 binds to the N-terminal part of ASK1 and blocks activation of ASK1 by TNF. 7,9  Neither the oxidized form (intramolecular disulfide between C32 and C35) nor the redox-inactive form (the double-mutation at catalytic sites C32 and C35) of Trx1 binds to ASK1.	bind
36818	6	8613	5	13	NULL	NULL	NULL	Trx1	GP	oxidized form	contains							intramolecular disulfide between	C32 and C35		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1483_s_39	15117824	7 Interestingly, only the reduced form of Trx1 binds to the N-terminal part of ASK1 and blocks activation of ASK1 by TNF. 7,9  Neither the oxidized form (intramolecular disulfide between C32 and C35) nor the redox-inactive form (the double-mutation at catalytic sites C32 and C35) of Trx1 binds to ASK1.	bind
36819	7	8613	5	13	NULL	NULL	NULL	Trx1	GP	redox-inactive form	contains							double-mutation at	catalytic sites C32;;C35		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1483_s_39	15117824	7 Interestingly, only the reduced form of Trx1 binds to the N-terminal part of ASK1 and blocks activation of ASK1 by TNF. 7,9  Neither the oxidized form (intramolecular disulfide between C32 and C35) nor the redox-inactive form (the double-mutation at catalytic sites C32 and C35) of Trx1 binds to ASK1.	bind
35936	1	8613	7	NULL	NULL	0	NULL	Trx1	NULL	reduced	binds to	NULL				ASK1	NULL		 N-terminal part		NULL		0	NULL	NULL	NULL	gw70_circulationres_94_11_1483_s_39	15117824	7 Interestingly, only the reduced form of Trx1 binds to the N-terminal part of ASK1 and blocks activation of ASK1 by TNF. 7,9  Neither the oxidized form (intramolecular disulfide between C32 and C35) nor the redox-inactive form (the double-mutation at catalytic sites C32 and C35) of Trx1 binds to ASK1.	bind
35937	2	8613	7	NULL	NULL	0	NULL	TNF	NULL		activates	NULL				ASK1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_11_1483_s_39	15117824	7 Interestingly, only the reduced form of Trx1 binds to the N-terminal part of ASK1 and blocks activation of ASK1 by TNF. 7,9  Neither the oxidized form (intramolecular disulfide between C32 and C35) nor the redox-inactive form (the double-mutation at catalytic sites C32 and C35) of Trx1 binds to ASK1.	bind
35938	3	8613	7	NULL	NULL	0	NULL	statement 1	NULL		blocks	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_11_1483_s_39	15117824	7 Interestingly, only the reduced form of Trx1 binds to the N-terminal part of ASK1 and blocks activation of ASK1 by TNF. 7,9  Neither the oxidized form (intramolecular disulfide between C32 and C35) nor the redox-inactive form (the double-mutation at catalytic sites C32 and C35) of Trx1 binds to ASK1.	bind
35939	4	8613	7	NULL	NULL	0	NULL	Trx1	NULL	Oxidized form	does not bind	NULL				ASK1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_11_1483_s_39	15117824	7 Interestingly, only the reduced form of Trx1 binds to the N-terminal part of ASK1 and blocks activation of ASK1 by TNF. 7,9  Neither the oxidized form (intramolecular disulfide between C32 and C35) nor the redox-inactive form (the double-mutation at catalytic sites C32 and C35) of Trx1 binds to ASK1.	bind
35940	5	8613	7	NULL	NULL	0	NULL	Trx1	NULL	 redox-inactive form	does not bind	NULL				ASK1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_11_1483_s_39	15117824	7 Interestingly, only the reduced form of Trx1 binds to the N-terminal part of ASK1 and blocks activation of ASK1 by TNF. 7,9  Neither the oxidized form (intramolecular disulfide between C32 and C35) nor the redox-inactive form (the double-mutation at catalytic sites C32 and C35) of Trx1 binds to ASK1.	bind
35941	6	8613	7	10	NULL	0	NULL	Trx1	NULL	oxidized form	contains	NULL				C32 and C35	NULL	intramolecular disulfide between			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1483_s_39	15117824	7 Interestingly, only the reduced form of Trx1 binds to the N-terminal part of ASK1 and blocks activation of ASK1 by TNF. 7,9  Neither the oxidized form (intramolecular disulfide between C32 and C35) nor the redox-inactive form (the double-mutation at catalytic sites C32 and C35) of Trx1 binds to ASK1.	bind
35942	7	8613	7	10	NULL	0	NULL	Trx1	NULL	oxidized form	contains	NULL				C32 and C35	NULL	double-mutation at catalytic sites			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_11_1483_s_39	15117824	7 Interestingly, only the reduced form of Trx1 binds to the N-terminal part of ASK1 and blocks activation of ASK1 by TNF. 7,9  Neither the oxidized form (intramolecular disulfide between C32 and C35) nor the redox-inactive form (the double-mutation at catalytic sites C32 and C35) of Trx1 binds to ASK1.	bind
36820	1	8614	5	13	NULL	NULL	NULL	Msx-1	GP		contains				promoter	Msx-1	GP			consensus binding sites	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_36_22667_s_260	9278425	7 Msx-1 promoter itself contains two  Msx-1 consensus binding sites and the binding of  Msx-1 homeodomain polypeptide to the predicted  Msx-1 motif was previously demonstrated ( 43).	bind
36821	2	8614	5	13	NULL	NULL	NULL	Msx-1 homeodomain polypeptide	GP		bind					Msx-1 motif	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_36_22667_s_260	9278425	7 Msx-1 promoter itself contains two  Msx-1 consensus binding sites and the binding of  Msx-1 homeodomain polypeptide to the predicted  Msx-1 motif was previously demonstrated ( 43).	bind
35943	1	8614	7	NULL	NULL	0	NULL	Msx-1	NULL		contains	NULL			promoter	Msx-1	NULL		consensus binding sites		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_36_22667_s_260	9278425	7 Msx-1 promoter itself contains two  Msx-1 consensus binding sites and the binding of  Msx-1 homeodomain polypeptide to the predicted  Msx-1 motif was previously demonstrated ( 43).	bind
35944	2	8614	7	NULL	NULL	0	NULL	Msx-1 homeodomain polypeptide	NULL		binds to	NULL				predicted Msx-1	NULL		motif		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_36_22667_s_260	9278425	7 Msx-1 promoter itself contains two  Msx-1 consensus binding sites and the binding of  Msx-1 homeodomain polypeptide to the predicted  Msx-1 motif was previously demonstrated ( 43).	bind
36822	1	8615	5	13	NULL	NULL	NULL	Pepf gene	GP		is expressed in					ZCs	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
36823	2	8615	5	13	NULL	NULL	NULL	Pepf	GP		is					pepsinogen F	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
36824	3	8615	5	13	NULL	NULL	NULL	Cckar gene	GP		is expressed in					ZCs	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
36825	4	8615	5	13	NULL	NULL	NULL	Cckar	GP		is					cholecystokinin receptor A	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
36826	5	8615	5	13	NULL	NULL	NULL	Cckar	GP		bind					cholecystokinin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
36827	6	8615	5	13	NULL	NULL	NULL	Cckar	GP		regulates					pepsinogen	GP	secretion of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
36828	7	8615	5	13	NULL	NULL	NULL	Amy2 gene	GP		is expressed in					ZCs	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
36829	8	8615	5	13	NULL	NULL	NULL	Amy2	GP		is					alpha-amylase	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
36830	9	8615	5	13	NULL	NULL	NULL	Try2/4 gene	GP		is expressed in					ZCs	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
36831	10	8615	5	13	NULL	NULL	NULL	Try2/4	GP		is					trypsin 2/4	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
36832	11	8615	5	13	NULL	NULL	NULL	Gif gene	GP		is expressed in					ZCs	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
36833	12	8615	5	13	NULL	NULL	NULL	Gif	GP		is					gastric intrinsic factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
36834	13	8615	5	13	NULL	NULL	NULL	Anpep gene	GP		is expressed in					ZCs	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
36835	14	8615	5	13	NULL	NULL	NULL	Anpep	GP		is					alanyl aminopeptidase N	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
36836	15	8615	5	13	NULL	NULL	NULL	Anpep	GP		also known as					CD13	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
36837	16	8615	5	13	NULL	NULL	NULL	Anpep	GP		is a type of					metalloproteinase	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
36838	17	8615	5	13	NULL	NULL	NULL	Anpep	GP		is present in					ZC vesicles	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
36839	18	8615	5	13	NULL	NULL	NULL	Spp1 gene	GP		is expressed in					ZCs	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
36840	19	8615	5	13	NULL	NULL	NULL	Spp1	GP		is					secreted phosphoprotein 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
36841	20	8615	5	13	NULL	NULL	NULL	Spp1	GP		also known as					osteopontin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
36842	21	8615	5	13	NULL	NULL	NULL	Spp1	GP		is a type of					adhesive glycoprotein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
36843	22	8615	5	13	NULL	NULL	NULL	Spp1	GP		is implicated in					mucosal barrier function	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
35945	1	8615	7	NULL	NULL	0	NULL	Pepf 	NULL		is	NULL				pepsinogen F	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
35946	3	8615	7	NULL	NULL	0	NULL	cholecystokinin	NULL		bind	NULL				cholecystokinin receptor A	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
35947	4	8615	7	NULL	NULL	0	NULL	statement 2	NULL		regulates	NULL				pepsinogen 	NULL	secretion of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
35949	2	8615	7	NULL	NULL	0	NULL	Pepf	NULL		is expressed in	NULL				ZCs	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
35950	5	8615	7	NULL	NULL	0	NULL	Cckar	NULL		is	NULL				cholecystokinin receptor A	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
35951	6	8615	7	NULL	NULL	0	NULL	Cckar	NULL		is expressed in	NULL				ZCs	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
35952	7	8615	7	NULL	NULL	0	NULL	Amy2	NULL		is	NULL				alpha-amylase	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
35953	8	8615	7	NULL	NULL	0	NULL	Amy2	NULL		is expressed in	NULL				ZCs	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
35954	9	8615	7	NULL	NULL	0	NULL	Try2/4 	NULL		is	NULL				trypsin 2/4	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
35955	10	8615	7	NULL	NULL	0	NULL	Try2/4 	NULL		is expressed in	NULL				ZCs	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
35956	11	8615	7	NULL	NULL	0	NULL	Gif	NULL		is	NULL				gastric intrinsic factor	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
35957	12	8615	7	NULL	NULL	0	NULL	Gif	NULL		is involved in	NULL				cobalamin	NULL	intestinal absorption of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
35958	13	8615	7	NULL	NULL	0	NULL	Gif	NULL		is expressed in	NULL				ZCs	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
35959	14	8615	7	NULL	NULL	0	NULL	Anpep 	NULL		is	NULL				alanyl aminopeptidase N	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
35960	15	8615	7	NULL	NULL	0	NULL	Anpep	NULL		is known as	NULL				CD13	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
35961	16	8615	7	NULL	NULL	0	NULL	Anpep	NULL		is a type of	NULL				metalloproteinase	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
35962	17	8615	7	NULL	NULL	0	NULL	Anpep	NULL		is found in	NULL				ZC vesicles	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
35963	18	8615	7	NULL	NULL	0	NULL	Spp1 	NULL		is	NULL				secreted phosphoprotein 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
35964	19	8615	7	NULL	NULL	0	NULL	Spp1 	NULL		is also known as	NULL				osteopontin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
35974	20	8615	7	NULL	NULL	0	NULL	Spp1	NULL		is a type of	NULL				adhesive glycoprotein	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
35976	21	8615	7	NULL	NULL	0	NULL	Spp1	NULL		is implicated in	NULL				mucosal barrier function	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
35978	22	8615	7	NULL	NULL	0	NULL	Spp1	NULL		is expressed in	NULL				ZCs	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46138_s_135	12963718	7 of the 12 genes were known to be expressed in ZCs:  Pepf (pepsinogen F, see Ref.  );  Cckar (cholecystokinin receptor A, binds cholecystokinin and is involved in regulating pepsinogen secretion) ( );  Amy2 (alpha-amylase);  Try2/4 (trypsin 2/4);  Gif (gastric intrinsic factor, intestinal absorption of cobalamin);  Anpep (alanyl aminopeptidase N, also known as CD13, a metalloproteinase found in ZC vesicles, see Ref.  ); and  Spp1 (secreted phosphoprotein 1 or osteopontin, an adhesive glycoprotein implicated in mucosal barrier function, Ref.  ).	bind
36844	1	8616	5	13	NULL	NULL	NULL	Rab3A	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_163_3_889_s_15	12937130	7 Rabphilin-3A binds to Rab3A only in its GTP-bound state, and the complex is required for the correct docking of synaptic vesicles to their target membrane.	bind
36845	2	8616	5	13	NULL	NULL	NULL	Rabphilin-3A	GP		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_163_3_889_s_15	12937130	7 Rabphilin-3A binds to Rab3A only in its GTP-bound state, and the complex is required for the correct docking of synaptic vesicles to their target membrane.	bind
36846	3	8616	5	13	NULL	NULL	NULL	synaptic vesicles	OrganismPart		is docked to					target membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_163_3_889_s_15	12937130	7 Rabphilin-3A binds to Rab3A only in its GTP-bound state, and the complex is required for the correct docking of synaptic vesicles to their target membrane.	bind
36847	4	8616	5	13	NULL	NULL	NULL	statement 2	Process		is required for					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_163_3_889_s_15	12937130	7 Rabphilin-3A binds to Rab3A only in its GTP-bound state, and the complex is required for the correct docking of synaptic vesicles to their target membrane.	bind
35986	1	8616	7	10	NULL	0	NULL	Rab3A			bind					GTP					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_163_3_889_s_15	12937130	7 Rabphilin-3A binds to Rab3A only in its GTP-bound state, and the complex is required for the correct docking of synaptic vesicles to their target membrane.	bind
35987	2	8616	7	10	NULL	0	NULL	Rabphilin-3A			bind					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_163_3_889_s_15	12937130	7 Rabphilin-3A binds to Rab3A only in its GTP-bound state, and the complex is required for the correct docking of synaptic vesicles to their target membrane.	bind
35988	3	8616	7	NULL	NULL	0	NULL	synaptic vesicles	NULL		docked to	NULL				target membrane	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_163_3_889_s_15	12937130	7 Rabphilin-3A binds to Rab3A only in its GTP-bound state, and the complex is required for the correct docking of synaptic vesicles to their target membrane.	bind
35991	4	8616	7	NULL	NULL	0	NULL	statement 1	NULL		is required for	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_163_3_889_s_15	12937130	7 Rabphilin-3A binds to Rab3A only in its GTP-bound state, and the complex is required for the correct docking of synaptic vesicles to their target membrane.	bind
36848	1	8617	5	13	NULL	NULL	NULL	RWJ-54428	Chemical		is a type of					parenteral cephalosporin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_49_5_845_s_48	12003982	7 RWJ-54428 is a parenteral cephalosporin that binds PBP2'' in staphylococci 5 and shows  in vitro activity against other Gram-positive bacteria, as well as  Haemophilus influenzae and  Moraxella catarrhalis.	bind
36849	2	8617	5	13	NULL	NULL	NULL	RWJ-54428	Chemical		bind					PBP2''	GP	staphylococci			NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_49_5_845_s_48	12003982	7 RWJ-54428 is a parenteral cephalosporin that binds PBP2'' in staphylococci 5 and shows  in vitro activity against other Gram-positive bacteria, as well as  Haemophilus influenzae and  Moraxella catarrhalis.	bind
36850	3	8617	5	13	NULL	NULL	NULL	RWJ-54428	Chemical		is active against					Gram-positive bacteria	Organism				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_49_5_845_s_48	12003982	7 RWJ-54428 is a parenteral cephalosporin that binds PBP2'' in staphylococci 5 and shows  in vitro activity against other Gram-positive bacteria, as well as  Haemophilus influenzae and  Moraxella catarrhalis.	bind
36851	4	8617	5	13	NULL	NULL	NULL	RWJ-54428	Chemical		is active against					Haemophilus influenzae	Organism				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_49_5_845_s_48	12003982	7 RWJ-54428 is a parenteral cephalosporin that binds PBP2'' in staphylococci 5 and shows  in vitro activity against other Gram-positive bacteria, as well as  Haemophilus influenzae and  Moraxella catarrhalis.	bind
36852	5	8617	5	13	NULL	NULL	NULL	RWJ-54428	Chemical		is active against					Moraxella catarrhalis	Organism				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_49_5_845_s_48	12003982	7 RWJ-54428 is a parenteral cephalosporin that binds PBP2'' in staphylococci 5 and shows  in vitro activity against other Gram-positive bacteria, as well as  Haemophilus influenzae and  Moraxella catarrhalis.	bind
35996	1	8617	7	NULL	NULL	0	NULL	RWJ-54428	NULL		is a type of	NULL				parenteral cephalosporin	NULL				NULL		0	NULL	NULL	NULL	gw60_jantimicrobchemoth_49_5_845_s_48	12003982	7 RWJ-54428 is a parenteral cephalosporin that binds PBP2'' in staphylococci 5 and shows  in vitro activity against other Gram-positive bacteria, as well as  Haemophilus influenzae and  Moraxella catarrhalis.	bind
35998	2	8617	7	10	NULL	0	NULL	RWJ-54428	NULL		binds	NULL				PBP2	NULL	staphylococci			NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_49_5_845_s_48	12003982	7 RWJ-54428 is a parenteral cephalosporin that binds PBP2'' in staphylococci 5 and shows  in vitro activity against other Gram-positive bacteria, as well as  Haemophilus influenzae and  Moraxella catarrhalis.	bind
36000	3	8617	7	10	NULL	0	NULL	RWJ-54428			is active against					Gram-positive bacteria					NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_49_5_845_s_48	12003982	7 RWJ-54428 is a parenteral cephalosporin that binds PBP2'' in staphylococci 5 and shows  in vitro activity against other Gram-positive bacteria, as well as  Haemophilus influenzae and  Moraxella catarrhalis.	bind
36001	4	8617	7	10	NULL	0	NULL	RWJ-54428			is active against					Haemophilus influenzae					NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_49_5_845_s_48	12003982	7 RWJ-54428 is a parenteral cephalosporin that binds PBP2'' in staphylococci 5 and shows  in vitro activity against other Gram-positive bacteria, as well as  Haemophilus influenzae and  Moraxella catarrhalis.	bind
36002	5	8617	7	10	NULL	0	NULL	RWJ-54428			is active against					Moraxella catarrhalis					NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_49_5_845_s_48	12003982	7 RWJ-54428 is a parenteral cephalosporin that binds PBP2'' in staphylococci 5 and shows  in vitro activity against other Gram-positive bacteria, as well as  Haemophilus influenzae and  Moraxella catarrhalis.	bind
36853	1	8618	5	13	NULL	NULL	NULL	WGA	GP		bind					alveolar epithelium	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jantimicrobchemoth_54_4_761_s_122	15329364	7 Sustained release of drugs upon administration of nebulized WGA-coated PLG-NPs indicates the binding of WGA on the alveolar epithelium.	bind
36003	1	8618	7	NULL	NULL	0	NULL	WGA	NULL		bind	NULL				alveolar epithelium	NULL				NULL		0	NULL	NULL	NULL	gw70_jantimicrobchemoth_54_4_761_s_122	15329364	7 Sustained release of drugs upon administration of nebulized WGA-coated PLG-NPs indicates the binding of WGA on the alveolar epithelium.	bind
37060	1	8619	5	13	NULL	NULL	NULL				bind		high affinity	extracellular domain of alpha subunit		PDGF-A chain	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2395_s_27	9409207	7 The extracellular domain of the alpha subunit binds both PDGF-A and -B chains with high affinity, whereas the beta subunit binds only the B-chain specifically.	bind
37061	2	8619	5	13	NULL	NULL	NULL				bind		high affinity	extracellular domain of alpha subunit		PDGF-B chain	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2395_s_27	9409207	7 The extracellular domain of the alpha subunit binds both PDGF-A and -B chains with high affinity, whereas the beta subunit binds only the B-chain specifically.	bind
37062	3	8619	5	13	NULL	NULL	NULL				bind		specifically	beta subunit		PDGF-B chain	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2395_s_27	9409207	7 The extracellular domain of the alpha subunit binds both PDGF-A and -B chains with high affinity, whereas the beta subunit binds only the B-chain specifically.	bind
36004	1	8619	7	NULL	NULL	0	NULL		NULL		bind	NULL	high affinity	extracellular domain of the alpha subunit 		PDGF	NULL		A chain		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2395_s_27	9409207	7 The extracellular domain of the alpha subunit binds both PDGF-A and -B chains with high affinity, whereas the beta subunit binds only the B-chain specifically.	bind
36005	2	8619	7	NULL	NULL	0	NULL		NULL		bind	NULL	high affinity	extracellular domain of the alpha subunit		PDGF	NULL		B chain		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2395_s_27	9409207	7 The extracellular domain of the alpha subunit binds both PDGF-A and -B chains with high affinity, whereas the beta subunit binds only the B-chain specifically.	bind
36006	3	8619	7	NULL	NULL	0	NULL		NULL		bind	NULL	specifically	beta subunit		B-chain	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2395_s_27	9409207	7 The extracellular domain of the alpha subunit binds both PDGF-A and -B chains with high affinity, whereas the beta subunit binds only the B-chain specifically.	bind
37063	1	8621	5	13	NULL	NULL	NULL	Chk1	GP	exogenous	bind					chromatin	Chromosome				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_27_25207_s_209	12676962	7 Therefore,  the amount of exogenous Chk1 bound to the chromatin argues against a  Chk1-EYFP-Chk1 dimer mechanism.	bind
36007	1	8621	7	NULL	NULL	0	NULL	Chk1	NULL	exogenous	bind	NULL				chromatin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_27_25207_s_209	12676962	7 Therefore,  the amount of exogenous Chk1 bound to the chromatin argues against a  Chk1-EYFP-Chk1 dimer mechanism.	bind
37705	1	8622	5	13	NULL	NULL	NULL	negatively charged groove	GP		attracts					positively charged surface	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_30_18849_s_130	9228061	7 This negatively charged groove could attract the positively charged surface formed by the putative adenylyl cyclase binding region of Gsalpha (alpha2/beta4 (switch 2), alpha3/beta5, and alpha4/beta6) ( 13,  14,  17) (Fig.  6,  B and  C).	bind
37706	2	8622	5	13	NULL	NULL	NULL	positively charged surface	GP		is formed by					Gsalpha	GP	putative 	adenylyl cyclase binding region		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_30_18849_s_130	9228061	7 This negatively charged groove could attract the positively charged surface formed by the putative adenylyl cyclase binding region of Gsalpha (alpha2/beta4 (switch 2), alpha3/beta5, and alpha4/beta6) ( 13,  14,  17) (Fig.  6,  B and  C).	bind
36008	1	8622	7	10	NULL	0	NULL	positively charged surface			is formed by					Gsalpha		putative	adenylyl cyclase binding region		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_30_18849_s_130	9228061	7 This negatively charged groove could attract the positively charged surface formed by the putative adenylyl cyclase binding region of Gsalpha (alpha2/beta4 (switch 2), alpha3/beta5, and alpha4/beta6) ( 13,  14,  17) (Fig.  6,  B and  C).	bind
46812	2	8622	7	10	NULL	0	NULL	 negatively charged groove 			attracts					positively charged surface					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_30_18849_s_130	9228061	7 This negatively charged groove could attract the positively charged surface formed by the putative adenylyl cyclase binding region of Gsalpha (alpha2/beta4 (switch 2), alpha3/beta5, and alpha4/beta6) ( 13,  14,  17) (Fig.  6,  B and  C).	bind
37065	1	8623	5	13	NULL	NULL	NULL	TIMPs	GP		bind					MMPs	GP	activated			NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_9_1166_s_266	15723986	7 TIMPs bind with activated MMPs in a 1:1 stoichiometric ratio and inhibit proteolytic activity.	bind
37066	2	8623	5	13	NULL	NULL	NULL	statement 1	GP		inhibit					proteolytic activity	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_111_9_1166_s_266	15723986	7 TIMPs bind with activated MMPs in a 1:1 stoichiometric ratio and inhibit proteolytic activity.	bind
36011	1	8623	7	NULL	NULL	0	NULL	TIMPs	NULL		bind	NULL				MMPs	NULL	activated			NULL		0	NULL	NULL	NULL	gw70_circulation_111_9_1166_s_266	15723986	7 TIMPs bind with activated MMPs in a 1:1 stoichiometric ratio and inhibit proteolytic activity.	bind
36012	2	8623	7	NULL	NULL	0	NULL	statement 1	NULL		inhibit	NULL				proteolytic activity	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_111_9_1166_s_266	15723986	7 TIMPs bind with activated MMPs in a 1:1 stoichiometric ratio and inhibit proteolytic activity.	bind
37067	1	8624	5	13	NULL	NULL	NULL	VWF	GP		is					von Willebrand factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_8_1360_s_26	12171801	7 We also tested the effects of the agent known to block von Willebrand factor (VWF) binding to platelet GP Ibalpha, which was reported to play crucial roles in platelet thrombus formation at sites exposed to high shear stress, 18 -  22 on platelet accumulation around stents.	bind
37068	2	8624	5	13	NULL	NULL	NULL	VWF	GP		bind					GP Ibalpha	GP	platelet			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_8_1360_s_26	12171801	7 We also tested the effects of the agent known to block von Willebrand factor (VWF) binding to platelet GP Ibalpha, which was reported to play crucial roles in platelet thrombus formation at sites exposed to high shear stress, 18 -  22 on platelet accumulation around stents.	bind
36013	1	8624	7	10	NULL	0	NULL	VWF			bind					GP Ibalpha		platelet			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_8_1360_s_26	12171801	7 We also tested the effects of the agent known to block von Willebrand factor (VWF) binding to platelet GP Ibalpha, which was reported to play crucial roles in platelet thrombus formation at sites exposed to high shear stress, 18 -  22 on platelet accumulation around stents.	bind
36014	2	8624	7	10	NULL	0	NULL	VWF			is					von Willebrand factor					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_8_1360_s_26	12171801	7 We also tested the effects of the agent known to block von Willebrand factor (VWF) binding to platelet GP Ibalpha, which was reported to play crucial roles in platelet thrombus formation at sites exposed to high shear stress, 18 -  22 on platelet accumulation around stents.	bind
37069	1	8625	5	13	NULL	NULL	NULL	dynamin	GP		bind		specifically			EHSH1	GP		C-terminal SH3 domains		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_26_18446_s_299	10373452	7) Binding of dynamin to EHSH1 was specific for three of the five C-terminal SH3 domains.	bind
36019	1	8625	7	10	NULL	0	NULL	dynamin 			bind		specifically			EHSH1			C-terminal SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_26_18446_s_299	10373452	7) Binding of dynamin to EHSH1 was specific for three of the five C-terminal SH3 domains.	bind
37070	1	8626	5	13	NULL	NULL	NULL	caveolin-1	GP		bind					eNOS	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_8_866_s_22	11988487	7, 12 -  16 With this in mind, a reasonable working model is that caveolin-1 binding to eNOS renders it less active.	bind
37071	2	8626	5	13	NULL	NULL	NULL	caveolin-1	GP		is rendered					less active	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_8_866_s_22	11988487	7, 12 -  16 With this in mind, a reasonable working model is that caveolin-1 binding to eNOS renders it less active.	bind
37072	3	8626	5	13	NULL	NULL	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_8_866_s_22	11988487	7, 12 -  16 With this in mind, a reasonable working model is that caveolin-1 binding to eNOS renders it less active.	bind
36029	1	8626	7	NULL	NULL	0	NULL	caveolin-1	NULL		bind	NULL				eNOS	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_8_866_s_22	11988487	7, 12 -  16 With this in mind, a reasonable working model is that caveolin-1 binding to eNOS renders it less active.	bind
36035	2	8626	7	NULL	NULL	0	NULL	eNOS	NULL		become	NULL				less active	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_8_866_s_22	11988487	7, 12 -  16 With this in mind, a reasonable working model is that caveolin-1 binding to eNOS renders it less active.	bind
36037	3	8626	7	NULL	NULL	0	NULL	statement 2	NULL		occurs upon	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_8_866_s_22	11988487	7, 12 -  16 With this in mind, a reasonable working model is that caveolin-1 binding to eNOS renders it less active.	bind
37073	1	8627	5	13	NULL	NULL	NULL	VEGF-C	GP		bind					VEGFR-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_893_s_17	11549582	7, 14  However, VEGF-C also binds VEGFR-2 (KDR), that is mainly expressed by activated endothelium of blood vessels, suggesting a potential function of VEGF-C in the induction of angiogenesis.	bind
37074	2	8627	5	13	NULL	NULL	NULL	VEGFR-2	GP		also known as					KDR	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_893_s_17	11549582	7, 14  However, VEGF-C also binds VEGFR-2 (KDR), that is mainly expressed by activated endothelium of blood vessels, suggesting a potential function of VEGF-C in the induction of angiogenesis.	bind
37075	3	8627	5	13	NULL	NULL	NULL	VEGFR-2	GP		is expressed by					endothelium of blood vessels	Cell	activated			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_893_s_17	11549582	7, 14  However, VEGF-C also binds VEGFR-2 (KDR), that is mainly expressed by activated endothelium of blood vessels, suggesting a potential function of VEGF-C in the induction of angiogenesis.	bind
37076	4	8627	5	13	NULL	NULL	NULL	VEGF-C	GP		induce		potentially			angiogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_893_s_17	11549582	7, 14  However, VEGF-C also binds VEGFR-2 (KDR), that is mainly expressed by activated endothelium of blood vessels, suggesting a potential function of VEGF-C in the induction of angiogenesis.	bind
37077	5	8627	5	13	NULL	NULL	NULL	statement 1	Process		suggest					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_3_893_s_17	11549582	7, 14  However, VEGF-C also binds VEGFR-2 (KDR), that is mainly expressed by activated endothelium of blood vessels, suggesting a potential function of VEGF-C in the induction of angiogenesis.	bind
36042	1	8627	7	NULL	NULL	0	NULL	VEGF-C	NULL		binds	NULL				KDR	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_3_893_s_17	11549582	7, 14  However, VEGF-C also binds VEGFR-2 (KDR), that is mainly expressed by activated endothelium of blood vessels, suggesting a potential function of VEGF-C in the induction of angiogenesis.	bind
36045	2	8627	7	NULL	NULL	0	NULL	KDR	NULL		is expressed in	NULL				endothelium of blood vessels	NULL	activated			NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_3_893_s_17	11549582	7, 14  However, VEGF-C also binds VEGFR-2 (KDR), that is mainly expressed by activated endothelium of blood vessels, suggesting a potential function of VEGF-C in the induction of angiogenesis.	bind
36047	3	8627	7	NULL	NULL	0	NULL	VEGF-C	NULL		induce	NULL				angiogenesis	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_3_893_s_17	11549582	7, 14  However, VEGF-C also binds VEGFR-2 (KDR), that is mainly expressed by activated endothelium of blood vessels, suggesting a potential function of VEGF-C in the induction of angiogenesis.	bind
36048	4	8627	7	NULL	NULL	0	NULL	statement 1	NULL		suggests	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_3_893_s_17	11549582	7, 14  However, VEGF-C also binds VEGFR-2 (KDR), that is mainly expressed by activated endothelium of blood vessels, suggesting a potential function of VEGF-C in the induction of angiogenesis.	bind
36049	5	8627	7	NULL	NULL	0	NULL	KDR	NULL		is	NULL				VEGFR-2	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_3_893_s_17	11549582	7, 14  However, VEGF-C also binds VEGFR-2 (KDR), that is mainly expressed by activated endothelium of blood vessels, suggesting a potential function of VEGF-C in the induction of angiogenesis.	bind
37078	1	8629	5	13	NULL	NULL	NULL	CRP	GP		bind					E-LDL	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_109_15_1870_s_162	15037531	7,8  CRP bound to E-LDL probably tempers terminal complement activation via the same mechanisms that have previously been delineated in other systems.	bind
37079	2	8629	5	13	NULL	NULL	NULL	statement 1	Process		temper					terminal complement	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_circulation_109_15_1870_s_162	15037531	7,8  CRP bound to E-LDL probably tempers terminal complement activation via the same mechanisms that have previously been delineated in other systems.	bind
36052	1	8629	7	NULL	NULL	0	NULL	CRP 	NULL		bind	NULL				E-LDL	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_109_15_1870_s_162	15037531	7,8  CRP bound to E-LDL probably tempers terminal complement activation via the same mechanisms that have previously been delineated in other systems.	bind
36053	2	8629	7	NULL	NULL	0	NULL	statement 1	NULL		tempers	NULL				complement	NULL	activation of	terminal		NULL		0	NULL	NULL	NULL	gw70_circulation_109_15_1870_s_162	15037531	7,8  CRP bound to E-LDL probably tempers terminal complement activation via the same mechanisms that have previously been delineated in other systems.	bind
37080	1	8630	5	13	NULL	NULL	NULL	cdk	GP		bind					cyclin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_5_501_s_21	12600884	7,8 Binding of the cdk to its specific cyclin leads to partial kinase activity, but full activity occurs only after phosphorylation by the cdk activating kinase (CAK).	bind
37081	2	8630	5	13	NULL	NULL	NULL	cdk	GP		exhibits					kinase activity	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_5_501_s_21	12600884	7,8 Binding of the cdk to its specific cyclin leads to partial kinase activity, but full activity occurs only after phosphorylation by the cdk activating kinase (CAK).	bind
37082	3	8630	5	13	NULL	NULL	NULL	CAK	GP		is					cdk activating kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_5_501_s_21	12600884	7,8 Binding of the cdk to its specific cyclin leads to partial kinase activity, but full activity occurs only after phosphorylation by the cdk activating kinase (CAK).	bind
37218	4	8630	5	13	NULL	NULL	NULL	CAK	GP		phosphorylate					cdk	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_5_501_s_21	12600884	7,8 Binding of the cdk to its specific cyclin leads to partial kinase activity, but full activity occurs only after phosphorylation by the cdk activating kinase (CAK).	bind
37219	5	8630	5	13	NULL	NULL	NULL	statement 4	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_5_501_s_21	12600884	7,8 Binding of the cdk to its specific cyclin leads to partial kinase activity, but full activity occurs only after phosphorylation by the cdk activating kinase (CAK).	bind
46711	6	8630	5	13	NULL	NULL	NULL	statement 1	Process		leads to					statement 2	Process	partial			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_5_501_s_21	12600884	7,8 Binding of the cdk to its specific cyclin leads to partial kinase activity, but full activity occurs only after phosphorylation by the cdk activating kinase (CAK).	bind
36054	1	8630	7	NULL	NULL	0	NULL	 cdk	NULL		bind	NULL				cyclin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_92_5_501_s_21	12600884	7,8 Binding of the cdk to its specific cyclin leads to partial kinase activity, but full activity occurs only after phosphorylation by the cdk activating kinase (CAK).	bind
36055	2	8630	7	10	NULL	0	NULL	cdk	NULL		exhibits	NULL				kinase activity	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_5_501_s_21	12600884	7,8 Binding of the cdk to its specific cyclin leads to partial kinase activity, but full activity occurs only after phosphorylation by the cdk activating kinase (CAK).	bind
36056	3	8630	7	10	NULL	0	NULL	CAK	NULL		phosphorylate	NULL				Cdk	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_5_501_s_21	12600884	7,8 Binding of the cdk to its specific cyclin leads to partial kinase activity, but full activity occurs only after phosphorylation by the cdk activating kinase (CAK).	bind
36057	4	8630	7	10	NULL	0	NULL	statement 3	NULL		leads to	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_92_5_501_s_21	12600884	7,8 Binding of the cdk to its specific cyclin leads to partial kinase activity, but full activity occurs only after phosphorylation by the cdk activating kinase (CAK).	bind
36058	5	8630	7	NULL	NULL	0	NULL	CAK	NULL		is	NULL				cdk activating kinase	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_92_5_501_s_21	12600884	7,8 Binding of the cdk to its specific cyclin leads to partial kinase activity, but full activity occurs only after phosphorylation by the cdk activating kinase (CAK).	bind
46713	6	8630	7	10	NULL	0	NULL	statement 1	NULL		leads to	NULL				statement 2	NULL	partial			NULL		0	NULL	NULL	NULL	gw60_circulationres_92_5_501_s_21	12600884	7,8 Binding of the cdk to its specific cyclin leads to partial kinase activity, but full activity occurs only after phosphorylation by the cdk activating kinase (CAK).	bind
37220	1	8631	5	13	NULL	NULL	NULL	BPDE-I	Chemical		is					7,8-Dihydroxy-9,10-epoxy-7,8,9,10-tetrahydrobenzo[a]pyrene	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_carcinogenesis_21_4_629_s_4	10753196	7,8-Dihydroxy-9,10-epoxy-7,8,9,10-tetrahydrobenzo[ apyrene(BPDE-I), an ultimate carcinogenic form of B[ aP, was covalently bound to triglyceride (TG).	bind
37221	2	8631	5	13	NULL	NULL	NULL	BPDE-I	Chemical		is a type of					ultimate carcinogenic form of B[a]P	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_carcinogenesis_21_4_629_s_4	10753196	7,8-Dihydroxy-9,10-epoxy-7,8,9,10-tetrahydrobenzo[ apyrene(BPDE-I), an ultimate carcinogenic form of B[ aP, was covalently bound to triglyceride (TG).	bind
37222	3	8631	5	13	NULL	NULL	NULL	BPDE-I	GP		bind		covalently			TG	GP				NULL		NULL	NULL	NULL	NULL	gw60_carcinogenesis_21_4_629_s_4	10753196	7,8-Dihydroxy-9,10-epoxy-7,8,9,10-tetrahydrobenzo[ apyrene(BPDE-I), an ultimate carcinogenic form of B[ aP, was covalently bound to triglyceride (TG).	bind
37223	4	8631	5	13	NULL	NULL	NULL	TG	Chemical		is					triglyceride	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_carcinogenesis_21_4_629_s_4	10753196	7,8-Dihydroxy-9,10-epoxy-7,8,9,10-tetrahydrobenzo[ apyrene(BPDE-I), an ultimate carcinogenic form of B[ aP, was covalently bound to triglyceride (TG).	bind
36059	1	8631	7	NULL	NULL	0	NULL	BPDE-I	NULL		bind	NULL	covalently			TG	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_21_4_629_s_4	10753196	7,8-Dihydroxy-9,10-epoxy-7,8,9,10-tetrahydrobenzo[ apyrene(BPDE-I), an ultimate carcinogenic form of B[ aP, was covalently bound to triglyceride (TG).	bind
36060	2	8631	7	NULL	NULL	0	NULL	BPDE-I	NULL		is	NULL				7,8-Dihydroxy-9,10-epoxy-7,8,9,10-tetrahydrobenzo[ apyrene	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_21_4_629_s_4	10753196	7,8-Dihydroxy-9,10-epoxy-7,8,9,10-tetrahydrobenzo[ apyrene(BPDE-I), an ultimate carcinogenic form of B[ aP, was covalently bound to triglyceride (TG).	bind
36061	3	8631	7	NULL	NULL	0	NULL	TG	NULL		is	NULL				triglyceride 	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_21_4_629_s_4	10753196	7,8-Dihydroxy-9,10-epoxy-7,8,9,10-tetrahydrobenzo[ apyrene(BPDE-I), an ultimate carcinogenic form of B[ aP, was covalently bound to triglyceride (TG).	bind
36062	4	8631	7	NULL	NULL	0	NULL	BPDE-I	NULL		is a type of	NULL				 carcinogenic form of B[ aP	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_21_4_629_s_4	10753196	7,8-Dihydroxy-9,10-epoxy-7,8,9,10-tetrahydrobenzo[ apyrene(BPDE-I), an ultimate carcinogenic form of B[ aP, was covalently bound to triglyceride (TG).	bind
37224	1	8632	5	13	NULL	NULL	NULL	7,8-S-OctaF7	Chemical		complex with					FGFR2IIIb	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_21052_s_94	16728399	7,8-S-OctaF7 forms complexes with FGFR2IIIb that bind FGF7 to form FGF7-(7,8-S-OctaF7)-FGFR2IIIb complexes with high specificity and specific activity relative to octasaccharides with lower affinity for FGF7 ( ).	bind
37225	2	8632	5	13	NULL	NULL	NULL	statement 1	GP		bind					FGF7	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_21052_s_94	16728399	7,8-S-OctaF7 forms complexes with FGFR2IIIb that bind FGF7 to form FGF7-(7,8-S-OctaF7)-FGFR2IIIb complexes with high specificity and specific activity relative to octasaccharides with lower affinity for FGF7 ( ).	bind
37226	3	8632	5	13	NULL	NULL	NULL	statement 2	GP		forms		high specificity			FGF7-(7,8-S-OctaF7)-FGFR2IIIb complexes	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_21052_s_94	16728399	7,8-S-OctaF7 forms complexes with FGFR2IIIb that bind FGF7 to form FGF7-(7,8-S-OctaF7)-FGFR2IIIb complexes with high specificity and specific activity relative to octasaccharides with lower affinity for FGF7 ( ).	bind
37227	4	8632	5	13	NULL	NULL	NULL	FGF7-(7,8-S-OctaF7)-FGFR2IIIb complexes	GP	specific activity of	is relative to					octasaccharides	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_21052_s_94	16728399	7,8-S-OctaF7 forms complexes with FGFR2IIIb that bind FGF7 to form FGF7-(7,8-S-OctaF7)-FGFR2IIIb complexes with high specificity and specific activity relative to octasaccharides with lower affinity for FGF7 ( ).	bind
37228	5	8632	5	13	NULL	NULL	NULL	octasaccharides	Chemical		affinity for		less			FGF7	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_21052_s_94	16728399	7,8-S-OctaF7 forms complexes with FGFR2IIIb that bind FGF7 to form FGF7-(7,8-S-OctaF7)-FGFR2IIIb complexes with high specificity and specific activity relative to octasaccharides with lower affinity for FGF7 ( ).	bind
36063	1	8632	7	NULL	NULL	0	NULL	7,8-S-OctaF7	NULL		complex with	NULL				FGFR2IIIb	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21052_s_94	16728399	7,8-S-OctaF7 forms complexes with FGFR2IIIb that bind FGF7 to form FGF7-(7,8-S-OctaF7)-FGFR2IIIb complexes with high specificity and specific activity relative to octasaccharides with lower affinity for FGF7 ( ).	bind
36064	2	8632	7	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL				FGF7	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21052_s_94	16728399	7,8-S-OctaF7 forms complexes with FGFR2IIIb that bind FGF7 to form FGF7-(7,8-S-OctaF7)-FGFR2IIIb complexes with high specificity and specific activity relative to octasaccharides with lower affinity for FGF7 ( ).	bind
36065	3	8632	7	NULL	NULL	0	NULL	statement 2	NULL		forms	NULL	high specificity			FGF7-(7,8-S-OctaF7)-FGFR2IIIb complexes 	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_21052_s_94	16728399	7,8-S-OctaF7 forms complexes with FGFR2IIIb that bind FGF7 to form FGF7-(7,8-S-OctaF7)-FGFR2IIIb complexes with high specificity and specific activity relative to octasaccharides with lower affinity for FGF7 ( ).	bind
36066	4	8632	7	NULL	NULL	0	NULL	octasaccharides 	NULL		affinity for	NULL	less			FGF7	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_21052_s_94	16728399	7,8-S-OctaF7 forms complexes with FGFR2IIIb that bind FGF7 to form FGF7-(7,8-S-OctaF7)-FGFR2IIIb complexes with high specificity and specific activity relative to octasaccharides with lower affinity for FGF7 ( ).	bind
36067	5	8632	7	NULL	NULL	0	NULL	statement 3	NULL		occurs with	NULL				specific activity	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21052_s_94	16728399	7,8-S-OctaF7 forms complexes with FGFR2IIIb that bind FGF7 to form FGF7-(7,8-S-OctaF7)-FGFR2IIIb complexes with high specificity and specific activity relative to octasaccharides with lower affinity for FGF7 ( ).	bind
37229	1	8633	5	13	NULL	NULL	NULL	ATP	Chemical		bind					P2Y receptors	GP				NULL	endothelium	NULL	NULL	NULL	NULL	gw70_circulationres_96_2_189_s_25	15604418	7,9  The released ATP then binds to P2Y receptors on the endothelium and stimulates vasodilatation by the release of nitric oxide (NO), prostaglandins, 2 and endothelium-derived hyperpolarizing factor (EDHF).	bind
37230	2	8633	5	13	NULL	NULL	NULL	statement 1	Process		stimulate					vasodilatation	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_2_189_s_25	15604418	7,9  The released ATP then binds to P2Y receptors on the endothelium and stimulates vasodilatation by the release of nitric oxide (NO), prostaglandins, 2 and endothelium-derived hyperpolarizing factor (EDHF).	bind
37231	3	8633	5	13	NULL	NULL	NULL	statement 2	Process		occurs by					NO	Chemical	release of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_2_189_s_25	15604418	7,9  The released ATP then binds to P2Y receptors on the endothelium and stimulates vasodilatation by the release of nitric oxide (NO), prostaglandins, 2 and endothelium-derived hyperpolarizing factor (EDHF).	bind
37232	4	8633	5	13	NULL	NULL	NULL	NO	Chemical		is					nitric oxide	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_2_189_s_25	15604418	7,9  The released ATP then binds to P2Y receptors on the endothelium and stimulates vasodilatation by the release of nitric oxide (NO), prostaglandins, 2 and endothelium-derived hyperpolarizing factor (EDHF).	bind
37233	5	8633	5	13	NULL	NULL	NULL	statement 2	Process		occurs by					prostaglandins	Chemical	release of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_2_189_s_25	15604418	7,9  The released ATP then binds to P2Y receptors on the endothelium and stimulates vasodilatation by the release of nitric oxide (NO), prostaglandins, 2 and endothelium-derived hyperpolarizing factor (EDHF).	bind
37234	6	8633	5	13	NULL	NULL	NULL	statement 2	Process		occurs by					EDHF	GP	release of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_2_189_s_25	15604418	7,9  The released ATP then binds to P2Y receptors on the endothelium and stimulates vasodilatation by the release of nitric oxide (NO), prostaglandins, 2 and endothelium-derived hyperpolarizing factor (EDHF).	bind
37235	7	8633	5	13	NULL	NULL	NULL	EDHF	GP		is					endothelium-derived hyperpolarizing factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_2_189_s_25	15604418	7,9  The released ATP then binds to P2Y receptors on the endothelium and stimulates vasodilatation by the release of nitric oxide (NO), prostaglandins, 2 and endothelium-derived hyperpolarizing factor (EDHF).	bind
36069	1	8633	7	NULL	NULL	0	NULL	ATP	NULL		binds	NULL				P2Y receptors	NULL				NULL	endothelium	0	NULL	NULL	NULL	gw70_circulationres_96_2_189_s_25	15604418	7,9  The released ATP then binds to P2Y receptors on the endothelium and stimulates vasodilatation by the release of nitric oxide (NO), prostaglandins, 2 and endothelium-derived hyperpolarizing factor (EDHF).	bind
36070	2	8633	7	NULL	NULL	0	NULL	statement 1	NULL		stimulates	NULL				vasodilatation	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_2_189_s_25	15604418	7,9  The released ATP then binds to P2Y receptors on the endothelium and stimulates vasodilatation by the release of nitric oxide (NO), prostaglandins, 2 and endothelium-derived hyperpolarizing factor (EDHF).	bind
36071	3	8633	7	NULL	NULL	0	NULL	statement 2	NULL		occurs by	NULL				NO	NULL	release of			NULL		0	NULL	NULL	NULL	gw70_circulationres_96_2_189_s_25	15604418	7,9  The released ATP then binds to P2Y receptors on the endothelium and stimulates vasodilatation by the release of nitric oxide (NO), prostaglandins, 2 and endothelium-derived hyperpolarizing factor (EDHF).	bind
36072	4	8633	7	NULL	NULL	0	NULL	statement 2	NULL		occurs by	NULL				prostaglandins	NULL	release of			NULL		0	NULL	NULL	NULL	gw70_circulationres_96_2_189_s_25	15604418	7,9  The released ATP then binds to P2Y receptors on the endothelium and stimulates vasodilatation by the release of nitric oxide (NO), prostaglandins, 2 and endothelium-derived hyperpolarizing factor (EDHF).	bind
36073	5	8633	7	NULL	NULL	0	NULL	statement 2	NULL		occurs by	NULL				EDHF	NULL	release of			NULL		0	NULL	NULL	NULL	gw70_circulationres_96_2_189_s_25	15604418	7,9  The released ATP then binds to P2Y receptors on the endothelium and stimulates vasodilatation by the release of nitric oxide (NO), prostaglandins, 2 and endothelium-derived hyperpolarizing factor (EDHF).	bind
36074	6	8633	7	NULL	NULL	0	NULL	NO	NULL		is	NULL				nitric oxide	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_2_189_s_25	15604418	7,9  The released ATP then binds to P2Y receptors on the endothelium and stimulates vasodilatation by the release of nitric oxide (NO), prostaglandins, 2 and endothelium-derived hyperpolarizing factor (EDHF).	bind
36075	7	8633	7	NULL	NULL	0	NULL	EDHF	NULL		is	NULL				endothelium-derived hyperpolarizing factor	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_2_189_s_25	15604418	7,9  The released ATP then binds to P2Y receptors on the endothelium and stimulates vasodilatation by the release of nitric oxide (NO), prostaglandins, 2 and endothelium-derived hyperpolarizing factor (EDHF).	bind
37236	1	8634	5	13	NULL	NULL	NULL	thrombin	GP		induce					SMCs	Cell	migration of;;rat			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
37237	2	8634	5	13	NULL	NULL	NULL	thrombin	GP		induce					SMCs	Cell	proliferation of;;rat			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
37238	3	8634	5	13	NULL	NULL	NULL	heparin	Chemical		inhibit		may;;partly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
37239	4	8634	5	13	NULL	NULL	NULL	heparin	Chemical		inhibit		may;;partly			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
37240	5	8634	5	13	NULL	NULL	NULL	HB-EGF	GP		bind					HSPGs	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
37241	6	8634	5	13	NULL	NULL	NULL	HSPGs	GP		is					heparan sulfate proteoglycans	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
37242	7	8634	5	13	NULL	NULL	NULL	heparin	Chemical		prevents					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
37243	8	8634	5	13	NULL	NULL	NULL	statement 7	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
37244	9	8634	5	13	NULL	NULL	NULL	statement 7	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
37245	10	8634	5	13	NULL	NULL	NULL	HB-EGF	GP		is a type of					heparin binding growth factors	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
37246	11	8634	5	13	NULL	NULL	NULL	bFGF	GP		is					basic fibroblast growth factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
37247	12	8634	5	13	NULL	NULL	NULL	bFGF	GP		is a type of					heparin binding growth factors	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
37248	13	8634	5	13	NULL	NULL	NULL	HSPGs	GP		acts as					coreceptors for biological activity	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
37249	14	8634	5	13	NULL	NULL	NULL	HB-EGF	GP		require					statement 13	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
37250	15	8634	5	13	NULL	NULL	NULL	bFGF	GP		requires					statement 13	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
36076	1	8634	7	10	NULL	0	NULL	thrombin			induce					SMCs		migration of;; rat			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
36077	2	8634	7	10	NULL	0	NULL	thrombin			induce					SMCs		proliferation of;; rat			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
36078	3	8634	7	NULL	NULL	0	NULL	heparin	NULL		inhibit	NULL	may			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
36079	4	8634	7	NULL	NULL	0	NULL	heparin	NULL		inhibit	NULL	may			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
36080	5	8634	7	NULL	NULL	0	NULL	HB-EGF	NULL		bind	NULL				HSPGs	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
36081	6	8634	7	NULL	NULL	0	NULL	HSPG	NULL		acts as	NULL				coreceptors	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
36082	7	8634	7	NULL	NULL	0	NULL	HB-EGF	NULL		requires	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
36083	8	8634	7	NULL	NULL	0	NULL	bFGF	NULL		requires	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
36084	9	8634	7	NULL	NULL	0	NULL	statement 3	NULL		occurs by	NULL				statement 5	NULL	prevention of			NULL		0	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
36085	10	8634	7	NULL	NULL	0	NULL	statement 4	NULL		occurs by	NULL				statement 5	NULL	prevention of			NULL		0	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
36087	11	8634	7	NULL	NULL	0	NULL	statement 9	NULL		because of	NULL				statement 7	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
36088	12	8634	7	NULL	NULL	0	NULL	statement 10	NULL		because of	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
36089	13	8634	7	NULL	NULL	0	NULL	HSPGs	NULL		is	NULL				heparan sulfate proteoglycans 	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
36090	14	8634	7	NULL	NULL	0	NULL	HB-EGF	NULL		is a type of	NULL				heparin binding growth factors	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
36091	15	8634	7	NULL	NULL	0	NULL	bFGF	NULL		is a type of	NULL				heparin binding growth factors	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
36092	16	8634	7	NULL	NULL	0	NULL	bFGF	NULL		is	NULL				basic fibroblast growth factor	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_2_172_s_20	15625285	7,9,10   Heparin may inhibit thrombin-induced migration and proliferation of rat SMCs, in part, by preventing the binding of HB-EGF to heparan sulfate proteoglycans (HSPGs), 7,11  because heparin binding growth factors (eg, HB-EGF, basic fibroblast growth factor [bFGF]) require HSPGs as coreceptors for biological activity.	bind
37888	1	8635	5	13	NULL	NULL	NULL	PDGF dimers	GP		bind					specific receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1763_s_16	10362801	7- 9  PDGF dimers bind to specific receptors that themselves are dimers formed from two types of subunits, alpha and beta, that differentially bind PDGF isoforms.	bind
37889	2	8635	5	13	NULL	NULL	NULL	PDGF receptors	GP		are					dimers	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1763_s_16	10362801	7- 9  PDGF dimers bind to specific receptors that themselves are dimers formed from two types of subunits, alpha and beta, that differentially bind PDGF isoforms.	bind
37890	3	8635	5	13	NULL	NULL	NULL	PDGF receptors	GP		are formed by								alpha and beta subunits		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1763_s_16	10362801	7- 9  PDGF dimers bind to specific receptors that themselves are dimers formed from two types of subunits, alpha and beta, that differentially bind PDGF isoforms.	bind
46716	4	8635	5	13	NULL	NULL	NULL	PDGF receptor	GP		bind		differentially			PDGF isoforms	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1763_s_16	10362801	7- 9  PDGF dimers bind to specific receptors that themselves are dimers formed from two types of subunits, alpha and beta, that differentially bind PDGF isoforms.	bind
36093	1	8635	7	NULL	NULL	0	NULL	PDGF dimers	NULL		bind	NULL				specific receptors	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1763_s_16	10362801	7- 9  PDGF dimers bind to specific receptors that themselves are dimers formed from two types of subunits, alpha and beta, that differentially bind PDGF isoforms.	bind
36094	4	8635	7	10	NULL	0	NULL	PDGF receptor	NULL		bind	NULL	differentially			PDGF isoforms	NULL				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_154_6_1763_s_16	10362801	7- 9  PDGF dimers bind to specific receptors that themselves are dimers formed from two types of subunits, alpha and beta, that differentially bind PDGF isoforms.	bind
37912	2	8635	7	NULL	NULL	0	NULL	PDGF receptors	NULL		are	NULL				dimers	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_6_1763_s_16	10362801	7- 9  PDGF dimers bind to specific receptors that themselves are dimers formed from two types of subunits, alpha and beta, that differentially bind PDGF isoforms.	bind
37913	3	8635	7	NULL	NULL	0	NULL	PDGF receptors	NULL		are formed by	NULL					NULL		alpha and beta subunit		NULL		0	NULL	NULL	NULL	gw60_amjpathol_154_6_1763_s_16	10362801	7- 9  PDGF dimers bind to specific receptors that themselves are dimers formed from two types of subunits, alpha and beta, that differentially bind PDGF isoforms.	bind
37252	1	8636	5	13	NULL	NULL	NULL	7-Deaza-cAMP	Chemical		bind					CRP	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1547_1_1_s_278	11343786	7-Deaza-cAMP binds to CRP, mediates a CRP conformation change, and promotes CRP-mediated  lacP activity in vivo and  catP activity in vitro to levels comparable to those attained with cAMP.	bind
37253	2	8636	5	13	NULL	NULL	NULL	statement 1	Process		mediate					CRP	GP	conformational changes in			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1547_1_1_s_278	11343786	7-Deaza-cAMP binds to CRP, mediates a CRP conformation change, and promotes CRP-mediated  lacP activity in vivo and  catP activity in vitro to levels comparable to those attained with cAMP.	bind
37254	3	8636	5	13	NULL	NULL	NULL	CRP	GP		mediate					lacP	GP	activity of			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1547_1_1_s_278	11343786	7-Deaza-cAMP binds to CRP, mediates a CRP conformation change, and promotes CRP-mediated  lacP activity in vivo and  catP activity in vitro to levels comparable to those attained with cAMP.	bind
37255	4	8636	5	13	NULL	NULL	NULL	statement 2	Process		promotes					statement 3	Process				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1547_1_1_s_278	11343786	7-Deaza-cAMP binds to CRP, mediates a CRP conformation change, and promotes CRP-mediated  lacP activity in vivo and  catP activity in vitro to levels comparable to those attained with cAMP.	bind
37256	5	8636	5	13	NULL	NULL	NULL	CRP	GP		mediate					catP	GP	activity of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1547_1_1_s_278	11343786	7-Deaza-cAMP binds to CRP, mediates a CRP conformation change, and promotes CRP-mediated  lacP activity in vivo and  catP activity in vitro to levels comparable to those attained with cAMP.	bind
37257	6	8636	5	13	NULL	NULL	NULL	statement 2	Process		promotes					statement 5	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1547_1_1_s_278	11343786	7-Deaza-cAMP binds to CRP, mediates a CRP conformation change, and promotes CRP-mediated  lacP activity in vivo and  catP activity in vitro to levels comparable to those attained with cAMP.	bind
36095	1	8636	7	NULL	NULL	0	NULL	7-Deaza-cAMP 	NULL		binds to	NULL				CRP	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1547_1_1_s_278	11343786	7-Deaza-cAMP binds to CRP, mediates a CRP conformation change, and promotes CRP-mediated  lacP activity in vivo and  catP activity in vitro to levels comparable to those attained with cAMP.	bind
36096	2	8636	7	NULL	NULL	0	NULL	statement 1	NULL		mediates	NULL				CRP	NULL	conformation change of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1547_1_1_s_278	11343786	7-Deaza-cAMP binds to CRP, mediates a CRP conformation change, and promotes CRP-mediated  lacP activity in vivo and  catP activity in vitro to levels comparable to those attained with cAMP.	bind
36097	3	8636	7	NULL	NULL	0	NULL	CRP	NULL		mediates	NULL				lacP activity	NULL				NULL	in vivo	0	NULL	NULL	NULL	gw60_biochimbiophysacta_1547_1_1_s_278	11343786	7-Deaza-cAMP binds to CRP, mediates a CRP conformation change, and promotes CRP-mediated  lacP activity in vivo and  catP activity in vitro to levels comparable to those attained with cAMP.	bind
36098	4	8636	7	NULL	NULL	0	NULL	statement 1	NULL		promotes	NULL				statement 3	NULL				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1547_1_1_s_278	11343786	7-Deaza-cAMP binds to CRP, mediates a CRP conformation change, and promotes CRP-mediated  lacP activity in vivo and  catP activity in vitro to levels comparable to those attained with cAMP.	bind
36099	5	8636	7	NULL	NULL	0	NULL	CRP	NULL		mediates	NULL				catP activity	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1547_1_1_s_278	11343786	7-Deaza-cAMP binds to CRP, mediates a CRP conformation change, and promotes CRP-mediated  lacP activity in vivo and  catP activity in vitro to levels comparable to those attained with cAMP.	bind
37908	6	8636	7	NULL	NULL	0	NULL	statement 1	NULL		promotes	NULL				statement 5	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1547_1_1_s_278	11343786	7-Deaza-cAMP binds to CRP, mediates a CRP conformation change, and promotes CRP-mediated  lacP activity in vivo and  catP activity in vitro to levels comparable to those attained with cAMP.	bind
37258	1	8637	5	13	NULL	NULL	NULL	RF	GP		bind					IgG	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_mol-immunol_32_1_7532785_s_8	7532785	7-mer  peptides representing RF-reactive sites on CH3 preincubated with polyclonal  IgM RF showed strong inhibition (55-66%) of RF binding to whole IgG on  the ELISA plate.	bind
37259	2	8637	5	13	NULL	NULL	NULL	7-mer peptides	GP		represents					CH3	GP		RF-reactive sites on		NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_mol-immunol_32_1_7532785_s_8	7532785	7-mer  peptides representing RF-reactive sites on CH3 preincubated with polyclonal  IgM RF showed strong inhibition (55-66%) of RF binding to whole IgG on  the ELISA plate.	bind
37260	3	8637	5	13	NULL	NULL	NULL	statement 2	Process		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_mol-immunol_32_1_7532785_s_8	7532785	7-mer  peptides representing RF-reactive sites on CH3 preincubated with polyclonal  IgM RF showed strong inhibition (55-66%) of RF binding to whole IgG on  the ELISA plate.	bind
36197	1	8637	7	NULL	NULL	0	NULL	RF	NULL		bind	NULL				IgG	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_mol-immunol_32_1_7532785_s_8	7532785	7-mer  peptides representing RF-reactive sites on CH3 preincubated with polyclonal  IgM RF showed strong inhibition (55-66%) of RF binding to whole IgG on  the ELISA plate.	bind
36198	2	8637	7	NULL	NULL	0	NULL	7-mer peptides	NULL		represent	NULL				CH3	NULL		RF-reactive sites		NULL		0	NULL	NULL	NULL	abs-batch0720-0739_mol-immunol_32_1_7532785_s_8	7532785	7-mer  peptides representing RF-reactive sites on CH3 preincubated with polyclonal  IgM RF showed strong inhibition (55-66%) of RF binding to whole IgG on  the ELISA plate.	bind
36199	3	8637	7	10	NULL	0	NULL	statement  2	NULL		inhibits	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_mol-immunol_32_1_7532785_s_8	7532785	7-mer  peptides representing RF-reactive sites on CH3 preincubated with polyclonal  IgM RF showed strong inhibition (55-66%) of RF binding to whole IgG on  the ELISA plate.	bind
37261	1	8638	5	13	NULL	NULL	NULL	7-methyl-GDP	Chemical		bind					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_89_6_951_s_123	9200613	7-methyl-GDP  binding to eIF4E Selected ligand atoms are labeled using lower case and italics  to distinguish them from protein components.	bind
36200	1	8638	7	NULL	NULL	0	NULL	7-methyl-GDP	NULL		bind	NULL				eIF4E	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_89_6_951_s_123	9200613	7-methyl-GDP  binding to eIF4E Selected ligand atoms are labeled using lower case and italics  to distinguish them from protein components.	bind
37262	1	8639	5	13	NULL	NULL	NULL	LD78	GP	receptor binding of	higher affinity than					MIP-1	GP	receptor binding of			NULL		NULL	NULL	NULL	NULL	gw60_febslett_457_2_219_s_69	10471782	70 ng/ml of MIP-1  was required for 50% inhibition of radiolabeled MIP-1  binding, while 20 ng/ml of LD78  was sufficient for 50% inhibition, indicating that LD78  has higher receptor binding affinity than MIP-1 .	bind
36201	1	8639	7	10	NULL	0	NULL	LD78	NULL	receptor binding of	higher affinity than	NULL				MIP-1	NULL	receptor binding of			NULL		NULL	NULL	NULL	NULL	gw60_febslett_457_2_219_s_69	10471782	70 ng/ml of MIP-1  was required for 50% inhibition of radiolabeled MIP-1  binding, while 20 ng/ml of LD78  was sufficient for 50% inhibition, indicating that LD78  has higher receptor binding affinity than MIP-1 .	bind
37263	1	8642	5	13	NULL	NULL	NULL	p53	GP		bind		sequence specifically			DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_5207_s_531	11812854	71       Hupp,T.R., Sparks,A. and Lane,D.P. (1995) Small peptides activate the latent sequence-specific DNA binding function of p53.	bind
37264	2	8642	5	13	NULL	NULL	NULL	peptides	GP	small	activates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_5207_s_531	11812854	71       Hupp,T.R., Sparks,A. and Lane,D.P. (1995) Small peptides activate the latent sequence-specific DNA binding function of p53.	bind
36207	1	8642	7	NULL	NULL	0	NULL	p53	NULL		bind	NULL	latent sequence-specific			DNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_5207_s_531	11812854	71       Hupp,T.R., Sparks,A. and Lane,D.P. (1995) Small peptides activate the latent sequence-specific DNA binding function of p53.	bind
36208	2	8642	7	NULL	NULL	0	NULL	Small peptides	NULL		activate	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_5207_s_531	11812854	71       Hupp,T.R., Sparks,A. and Lane,D.P. (1995) Small peptides activate the latent sequence-specific DNA binding function of p53.	bind
37707	1	8643	5	13	NULL	NULL	NULL	vitamin B12	Chemical		is a type of					Cbl III	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2074_s_30	9351374	71  Intracellularly, Cbl III (eg, vitamin B12, CN-Cbl) undergoes a beta-axial ligand exchange and cobalt reduction reactions catalyzed by the beta-axial ligand transferase/Cbl reductase complex to form Cbl II, which is initially bound to apo-methionine synthase.	bind
37708	2	8643	5	13	NULL	NULL	NULL	CN-Cbl	Chemical		is a type of					Cbl III	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2074_s_30	9351374	71  Intracellularly, Cbl III (eg, vitamin B12, CN-Cbl) undergoes a beta-axial ligand exchange and cobalt reduction reactions catalyzed by the beta-axial ligand transferase/Cbl reductase complex to form Cbl II, which is initially bound to apo-methionine synthase.	bind
37709	3	8643	5	13	NULL	NULL	NULL	Cbl III	Chemical		undergoes					beta-axial ligand exchange	Process				NULL	intracellularly	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2074_s_30	9351374	71  Intracellularly, Cbl III (eg, vitamin B12, CN-Cbl) undergoes a beta-axial ligand exchange and cobalt reduction reactions catalyzed by the beta-axial ligand transferase/Cbl reductase complex to form Cbl II, which is initially bound to apo-methionine synthase.	bind
37710	4	8643	5	13	NULL	NULL	NULL	Cbl III	Chemical		undergoes					cobalt reduction reactions	Process				NULL	intracellularly	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2074_s_30	9351374	71  Intracellularly, Cbl III (eg, vitamin B12, CN-Cbl) undergoes a beta-axial ligand exchange and cobalt reduction reactions catalyzed by the beta-axial ligand transferase/Cbl reductase complex to form Cbl II, which is initially bound to apo-methionine synthase.	bind
37711	5	8643	5	13	NULL	NULL	NULL	statement 3	Process		is catalyzed by					beta-axial ligand transferase/Cbl reductase complex	GP				NULL	intracellularly	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2074_s_30	9351374	71  Intracellularly, Cbl III (eg, vitamin B12, CN-Cbl) undergoes a beta-axial ligand exchange and cobalt reduction reactions catalyzed by the beta-axial ligand transferase/Cbl reductase complex to form Cbl II, which is initially bound to apo-methionine synthase.	bind
37712	6	8643	5	13	NULL	NULL	NULL	statement 4	Process		is catalyzed by					beta-axial ligand transferase/Cbl reductase complex	Process				NULL	intracellularly	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2074_s_30	9351374	71  Intracellularly, Cbl III (eg, vitamin B12, CN-Cbl) undergoes a beta-axial ligand exchange and cobalt reduction reactions catalyzed by the beta-axial ligand transferase/Cbl reductase complex to form Cbl II, which is initially bound to apo-methionine synthase.	bind
37713	7	8643	5	13	NULL	NULL	NULL	Cbl III	Chemical		forms					Cbl II	Chemical				NULL	intracellularly	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2074_s_30	9351374	71  Intracellularly, Cbl III (eg, vitamin B12, CN-Cbl) undergoes a beta-axial ligand exchange and cobalt reduction reactions catalyzed by the beta-axial ligand transferase/Cbl reductase complex to form Cbl II, which is initially bound to apo-methionine synthase.	bind
37714	8	8643	5	13	NULL	NULL	NULL	statement 3	Process		leads to					statement 7	Process				NULL	intracellularly	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2074_s_30	9351374	71  Intracellularly, Cbl III (eg, vitamin B12, CN-Cbl) undergoes a beta-axial ligand exchange and cobalt reduction reactions catalyzed by the beta-axial ligand transferase/Cbl reductase complex to form Cbl II, which is initially bound to apo-methionine synthase.	bind
37715	9	8643	5	13	NULL	NULL	NULL	statement 4	Process		leads to					statement 7	Process				NULL	intracellularly	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2074_s_30	9351374	71  Intracellularly, Cbl III (eg, vitamin B12, CN-Cbl) undergoes a beta-axial ligand exchange and cobalt reduction reactions catalyzed by the beta-axial ligand transferase/Cbl reductase complex to form Cbl II, which is initially bound to apo-methionine synthase.	bind
37716	10	8643	5	13	NULL	NULL	NULL	Cbl II	Chemical		bind		initially			apo-methionine synthase	GP				NULL	intracellularly	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2074_s_30	9351374	71  Intracellularly, Cbl III (eg, vitamin B12, CN-Cbl) undergoes a beta-axial ligand exchange and cobalt reduction reactions catalyzed by the beta-axial ligand transferase/Cbl reductase complex to form Cbl II, which is initially bound to apo-methionine synthase.	bind
36209	4	8643	7	NULL	NULL	0	NULL	Cbl III	NULL		forms	NULL				Cbl II	NULL				NULL	Intracellular	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2074_s_30	9351374	71  Intracellularly, Cbl III (eg, vitamin B12, CN-Cbl) undergoes a beta-axial ligand exchange and cobalt reduction reactions catalyzed by the beta-axial ligand transferase/Cbl reductase complex to form Cbl II, which is initially bound to apo-methionine synthase.	bind
36211	1	8643	7	NULL	NULL	0	NULL	Cbl II	NULL		bind	NULL				apo-methionine synthase	NULL				NULL	Intracellular	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2074_s_30	9351374	71  Intracellularly, Cbl III (eg, vitamin B12, CN-Cbl) undergoes a beta-axial ligand exchange and cobalt reduction reactions catalyzed by the beta-axial ligand transferase/Cbl reductase complex to form Cbl II, which is initially bound to apo-methionine synthase.	bind
36212	2	8643	7	NULL	NULL	0	NULL	Cbl III	NULL		undergoes	NULL				 beta-axial ligand exchange	NULL				NULL	Intracellular	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2074_s_30	9351374	71  Intracellularly, Cbl III (eg, vitamin B12, CN-Cbl) undergoes a beta-axial ligand exchange and cobalt reduction reactions catalyzed by the beta-axial ligand transferase/Cbl reductase complex to form Cbl II, which is initially bound to apo-methionine synthase.	bind
36213	3	8643	7	NULL	NULL	0	NULL	Cbl III	NULL		undergoes	NULL				cobalt reduction reactions	NULL				NULL	Intracellular	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2074_s_30	9351374	71  Intracellularly, Cbl III (eg, vitamin B12, CN-Cbl) undergoes a beta-axial ligand exchange and cobalt reduction reactions catalyzed by the beta-axial ligand transferase/Cbl reductase complex to form Cbl II, which is initially bound to apo-methionine synthase.	bind
36214	5	8643	7	NULL	NULL	0	NULL	beta-axial ligand transferase/Cbl reductase complex 	NULL		catalyse	NULL				statement 2	NULL				NULL	Intracellular	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2074_s_30	9351374	71  Intracellularly, Cbl III (eg, vitamin B12, CN-Cbl) undergoes a beta-axial ligand exchange and cobalt reduction reactions catalyzed by the beta-axial ligand transferase/Cbl reductase complex to form Cbl II, which is initially bound to apo-methionine synthase.	bind
36215	6	8643	7	NULL	NULL	0	NULL	beta-axial ligand transferase/Cbl reductase complex 	NULL		catalyse	NULL				statement 3	NULL				NULL	Intracellular	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2074_s_30	9351374	71  Intracellularly, Cbl III (eg, vitamin B12, CN-Cbl) undergoes a beta-axial ligand exchange and cobalt reduction reactions catalyzed by the beta-axial ligand transferase/Cbl reductase complex to form Cbl II, which is initially bound to apo-methionine synthase.	bind
36216	7	8643	7	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2074_s_30	9351374	71  Intracellularly, Cbl III (eg, vitamin B12, CN-Cbl) undergoes a beta-axial ligand exchange and cobalt reduction reactions catalyzed by the beta-axial ligand transferase/Cbl reductase complex to form Cbl II, which is initially bound to apo-methionine synthase.	bind
36217	8	8643	7	NULL	NULL	0	NULL	statement 3	NULL		leads to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2074_s_30	9351374	71  Intracellularly, Cbl III (eg, vitamin B12, CN-Cbl) undergoes a beta-axial ligand exchange and cobalt reduction reactions catalyzed by the beta-axial ligand transferase/Cbl reductase complex to form Cbl II, which is initially bound to apo-methionine synthase.	bind
36218	9	8643	7	NULL	NULL	0	NULL	vitamin B12	NULL		is a type of	NULL				Cbl III	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2074_s_30	9351374	71  Intracellularly, Cbl III (eg, vitamin B12, CN-Cbl) undergoes a beta-axial ligand exchange and cobalt reduction reactions catalyzed by the beta-axial ligand transferase/Cbl reductase complex to form Cbl II, which is initially bound to apo-methionine synthase.	bind
36219	10	8643	7	NULL	NULL	0	NULL	CN-Cbl	NULL		is a type of	NULL				Cbl III	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_10_2074_s_30	9351374	71  Intracellularly, Cbl III (eg, vitamin B12, CN-Cbl) undergoes a beta-axial ligand exchange and cobalt reduction reactions catalyzed by the beta-axial ligand transferase/Cbl reductase complex to form Cbl II, which is initially bound to apo-methionine synthase.	bind
37265	1	8644	5	13	NULL	NULL	NULL	estrogen receptor	GP		bind			DNA binding domain						estrogen response element	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_479	11452016	72       Romine,L.E., Wood,J.R., Lamia,L.A., Prendergast,P., Edwards,D.P. and Nardulli,A.M. (1998) The high mobility group protein 1 enhances binding of the estrogen receptor DNA binding domain to the estrogen response element.	bind
37266	2	8644	5	13	NULL	NULL	NULL	high mobility group protein 1	GP		enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_479	11452016	72       Romine,L.E., Wood,J.R., Lamia,L.A., Prendergast,P., Edwards,D.P. and Nardulli,A.M. (1998) The high mobility group protein 1 enhances binding of the estrogen receptor DNA binding domain to the estrogen response element.	bind
36220	1	8644	7	10	NULL	0	NULL	estrogen receptor			bind			DNA binding domain						estrogen response element	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_479	11452016	72       Romine,L.E., Wood,J.R., Lamia,L.A., Prendergast,P., Edwards,D.P. and Nardulli,A.M. (1998) The high mobility group protein 1 enhances binding of the estrogen receptor DNA binding domain to the estrogen response element.	bind
36221	2	8644	7	NULL	NULL	0	NULL	high mobility group protein 1	NULL		enhances	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_479	11452016	72       Romine,L.E., Wood,J.R., Lamia,L.A., Prendergast,P., Edwards,D.P. and Nardulli,A.M. (1998) The high mobility group protein 1 enhances binding of the estrogen receptor DNA binding domain to the estrogen response element.	bind
37267	1	8645	5	13	NULL	NULL	NULL	thrombin	GP		bind					GP Ib-IX-V complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_138	12231555	72 The binding of thrombin to the GP Ib-IX-V complex significantly enhances the ability of thrombin to cleave PAR1 and catalyze platelet activation.	bind
37268	2	8645	5	13	NULL	NULL	NULL	thrombin	GP		cleave					PAR1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_138	12231555	72 The binding of thrombin to the GP Ib-IX-V complex significantly enhances the ability of thrombin to cleave PAR1 and catalyze platelet activation.	bind
37269	3	8645	5	13	NULL	NULL	NULL	statement 2	Process		catalyze					platelet	Cell	activation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_138	12231555	72 The binding of thrombin to the GP Ib-IX-V complex significantly enhances the ability of thrombin to cleave PAR1 and catalyze platelet activation.	bind
37270	4	8645	5	13	NULL	NULL	NULL	statement 1	Process		enhance		significantly			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_138	12231555	72 The binding of thrombin to the GP Ib-IX-V complex significantly enhances the ability of thrombin to cleave PAR1 and catalyze platelet activation.	bind
37271	5	8645	5	13	NULL	NULL	NULL	statement 1	Process		enhance		significantly			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_138	12231555	72 The binding of thrombin to the GP Ib-IX-V complex significantly enhances the ability of thrombin to cleave PAR1 and catalyze platelet activation.	bind
36222	1	8645	7	NULL	NULL	0	NULL	thrombin	NULL		bind	NULL				GP Ib-IX-V complex	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_138	12231555	72 The binding of thrombin to the GP Ib-IX-V complex significantly enhances the ability of thrombin to cleave PAR1 and catalyze platelet activation.	bind
36223	2	8645	7	NULL	NULL	0	NULL	thrombin	NULL		cleave	NULL				PAR1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_138	12231555	72 The binding of thrombin to the GP Ib-IX-V complex significantly enhances the ability of thrombin to cleave PAR1 and catalyze platelet activation.	bind
36224	3	8645	7	NULL	NULL	0	NULL	thrombin	NULL		catalyze	NULL				platelet	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_138	12231555	72 The binding of thrombin to the GP Ib-IX-V complex significantly enhances the ability of thrombin to cleave PAR1 and catalyze platelet activation.	bind
36225	4	8645	7	NULL	NULL	0	NULL	statement 1	NULL		enhance	NULL	significantly			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_138	12231555	72 The binding of thrombin to the GP Ib-IX-V complex significantly enhances the ability of thrombin to cleave PAR1 and catalyze platelet activation.	bind
36226	5	8645	7	NULL	NULL	0	NULL	statement 1	NULL		enhance	NULL	significantly			statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_138	12231555	72 The binding of thrombin to the GP Ib-IX-V complex significantly enhances the ability of thrombin to cleave PAR1 and catalyze platelet activation.	bind
37272	1	8646	5	13	NULL	NULL	NULL	p53	GP		is a type of					T antigen binding proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_10_1044_s_132	12039793	72, 73 These studies revealed that 2 of T antigen binding proteins (namely p53 and p193) encode proapoptotic activity and suggested that minimally these 2 pathways must be circumvented to promote sustained cardiomyocyte proliferation.	bind
37273	2	8646	5	13	NULL	NULL	NULL	p193	GP		is a type of					T antigen binding proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_10_1044_s_132	12039793	72, 73 These studies revealed that 2 of T antigen binding proteins (namely p53 and p193) encode proapoptotic activity and suggested that minimally these 2 pathways must be circumvented to promote sustained cardiomyocyte proliferation.	bind
37274	3	8646	5	13	NULL	NULL	NULL	p53	GP		encode					proapoptotic activity	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_10_1044_s_132	12039793	72, 73 These studies revealed that 2 of T antigen binding proteins (namely p53 and p193) encode proapoptotic activity and suggested that minimally these 2 pathways must be circumvented to promote sustained cardiomyocyte proliferation.	bind
37275	4	8646	5	13	NULL	NULL	NULL	p193	GP		encode					proapoptotic activity	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_10_1044_s_132	12039793	72, 73 These studies revealed that 2 of T antigen binding proteins (namely p53 and p193) encode proapoptotic activity and suggested that minimally these 2 pathways must be circumvented to promote sustained cardiomyocyte proliferation.	bind
37276	5	8646	5	13	NULL	NULL	NULL	statement 3	Process		promotes					cardiomyocyte	Cell	proliferation of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_10_1044_s_132	12039793	72, 73 These studies revealed that 2 of T antigen binding proteins (namely p53 and p193) encode proapoptotic activity and suggested that minimally these 2 pathways must be circumvented to promote sustained cardiomyocyte proliferation.	bind
37277	6	8646	5	13	NULL	NULL	NULL	statement 4	Process		promotes					cardiomyocyte	Cell	proliferation of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_10_1044_s_132	12039793	72, 73 These studies revealed that 2 of T antigen binding proteins (namely p53 and p193) encode proapoptotic activity and suggested that minimally these 2 pathways must be circumvented to promote sustained cardiomyocyte proliferation.	bind
36227	1	8646	7	NULL	NULL	0	NULL	p53 	NULL		encode	NULL				proapoptotic activity	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_10_1044_s_132	12039793	72, 73 These studies revealed that 2 of T antigen binding proteins (namely p53 and p193) encode proapoptotic activity and suggested that minimally these 2 pathways must be circumvented to promote sustained cardiomyocyte proliferation.	bind
36228	2	8646	7	NULL	NULL	0	NULL	p193	NULL		encode	NULL				proapoptotic activity	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_10_1044_s_132	12039793	72, 73 These studies revealed that 2 of T antigen binding proteins (namely p53 and p193) encode proapoptotic activity and suggested that minimally these 2 pathways must be circumvented to promote sustained cardiomyocyte proliferation.	bind
36229	3	8646	7	NULL	NULL	0	NULL	statement 1	NULL		promote	NULL				cardiomyocytes	NULL	proliferation of 			NULL		0	NULL	NULL	NULL	gw60_circulationres_90_10_1044_s_132	12039793	72, 73 These studies revealed that 2 of T antigen binding proteins (namely p53 and p193) encode proapoptotic activity and suggested that minimally these 2 pathways must be circumvented to promote sustained cardiomyocyte proliferation.	bind
36230	4	8646	7	NULL	NULL	0	NULL	p53	NULL		is a type of	NULL				T antigen binding protein	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_10_1044_s_132	12039793	72, 73 These studies revealed that 2 of T antigen binding proteins (namely p53 and p193) encode proapoptotic activity and suggested that minimally these 2 pathways must be circumvented to promote sustained cardiomyocyte proliferation.	bind
36231	5	8646	7	NULL	NULL	0	NULL	p193	NULL		is a type of	NULL				T antigen binding protein	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_10_1044_s_132	12039793	72, 73 These studies revealed that 2 of T antigen binding proteins (namely p53 and p193) encode proapoptotic activity and suggested that minimally these 2 pathways must be circumvented to promote sustained cardiomyocyte proliferation.	bind
36232	6	8646	7	NULL	NULL	0	NULL	statement 2	NULL		promote	NULL				cardiomyocytes	NULL	proliferation of			NULL		0	NULL	NULL	NULL	gw60_circulationres_90_10_1044_s_132	12039793	72, 73 These studies revealed that 2 of T antigen binding proteins (namely p53 and p193) encode proapoptotic activity and suggested that minimally these 2 pathways must be circumvented to promote sustained cardiomyocyte proliferation.	bind
37278	1	8647	5	13	NULL	NULL	NULL	IgE	GP		bind		strongly			nLol p 5	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_462_3_435_s_130	10622741	72.7% of the patient sera showed strong IgE binding to nLol p 5 and rLol p 5C.	bind
37279	2	8647	5	13	NULL	NULL	NULL	IgE	GP		bind		strongly			rLol p 5C	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_462_3_435_s_130	10622741	72.7% of the patient sera showed strong IgE binding to nLol p 5 and rLol p 5C.	bind
36233	1	8647	7	NULL	NULL	0	NULL	 IgE	NULL		bind	NULL	strongly			nLol p 5 	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_462_3_435_s_130	10622741	72.7% of the patient sera showed strong IgE binding to nLol p 5 and rLol p 5C.	bind
36234	2	8647	7	NULL	NULL	0	NULL	IgE	NULL		bind	NULL	strongly			rLol p 5C	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_462_3_435_s_130	10622741	72.7% of the patient sera showed strong IgE binding to nLol p 5 and rLol p 5C.	bind
37280	1	8648	5	13	NULL	NULL	NULL	thrombin	GP		bind					GP Ib-IX-V complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_139	12231555	73 The binding of thrombin to the GP Ib-IX-V complex may also signal platelet activation through a fibrin-dependent mechanism.	bind
37281	2	8648	5	13	NULL	NULL	NULL	statement 1	Process		signal					platelet	Cell	activation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_139	12231555	73 The binding of thrombin to the GP Ib-IX-V complex may also signal platelet activation through a fibrin-dependent mechanism.	bind
37282	3	8648	5	13	NULL	NULL	NULL	statement 2	Process		through					fibrin-dependent mechanism	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_139	12231555	73 The binding of thrombin to the GP Ib-IX-V complex may also signal platelet activation through a fibrin-dependent mechanism.	bind
36235	1	8648	7	NULL	NULL	0	NULL	thrombin	NULL		bind	NULL				GP Ib-IX-V complex	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_139	12231555	73 The binding of thrombin to the GP Ib-IX-V complex may also signal platelet activation through a fibrin-dependent mechanism.	bind
36236	2	8648	7	NULL	NULL	0	NULL	statement 1	NULL		signal	NULL				platelet	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_139	12231555	73 The binding of thrombin to the GP Ib-IX-V complex may also signal platelet activation through a fibrin-dependent mechanism.	bind
36237	3	8648	7	NULL	NULL	0	NULL	statement 2	NULL		occurs through	NULL				fibrin-dependent mechanism	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_9_1381_s_139	12231555	73 The binding of thrombin to the GP Ib-IX-V complex may also signal platelet activation through a fibrin-dependent mechanism.	bind
37283	1	8649	5	13	NULL	NULL	NULL	HDL	GP		isolated from					atheroma	MedicalFinding	human			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1102_s_100	15790935	73,74  Moreover, HDL isolated from human atheroma contains MPO, consistent with the recent finding that MPO selectively binds to apolipoprotein A-I within plasma via a specific region on helix 8 of the lipoprotein.	bind
37284	2	8649	5	13	NULL	NULL	NULL	statement 1	GP		contains					MPO	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1102_s_100	15790935	73,74  Moreover, HDL isolated from human atheroma contains MPO, consistent with the recent finding that MPO selectively binds to apolipoprotein A-I within plasma via a specific region on helix 8 of the lipoprotein.	bind
37285	3	8649	5	13	NULL	NULL	NULL	MPO	GP		bind		selectively			apolipoprotein A-I	GP		helix 8		NULL	plasma	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1102_s_100	15790935	73,74  Moreover, HDL isolated from human atheroma contains MPO, consistent with the recent finding that MPO selectively binds to apolipoprotein A-I within plasma via a specific region on helix 8 of the lipoprotein.	bind
36238	1	8649	7	NULL	NULL	0	NULL	MPO	NULL		binds	NULL	selectively			apolipoprotein A-I 	NULL		helix 8		NULL	within plasma	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1102_s_100	15790935	73,74  Moreover, HDL isolated from human atheroma contains MPO, consistent with the recent finding that MPO selectively binds to apolipoprotein A-I within plasma via a specific region on helix 8 of the lipoprotein.	bind
36239	2	8649	7	NULL	NULL	0	NULL	HDL	NULL		contains	NULL				MPO	NULL				NULL	human atheroma	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_6_1102_s_100	15790935	73,74  Moreover, HDL isolated from human atheroma contains MPO, consistent with the recent finding that MPO selectively binds to apolipoprotein A-I within plasma via a specific region on helix 8 of the lipoprotein.	bind
37286	1	8650	5	13	NULL	NULL	NULL	estrogen receptor	GP		bind									estrogen response element	NULL	stably transfected HeLa cells	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_485	11452016	74       Zhang,C.C., Krieg,S. and Shapiro,D.J. (1999) HMG-1 stimulates estrogen response element binding by estrogen receptor from stably transfected HeLa cells.	bind
37287	2	8650	5	13	NULL	NULL	NULL	HMG-1	GP		stimulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_485	11452016	74       Zhang,C.C., Krieg,S. and Shapiro,D.J. (1999) HMG-1 stimulates estrogen response element binding by estrogen receptor from stably transfected HeLa cells.	bind
36240	1	8650	7	10	NULL	0	NULL	estrogen receptor	NULL		bind	NULL					NULL			estrogen response element	NULL	transfected HeLa cells	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_485	11452016	74       Zhang,C.C., Krieg,S. and Shapiro,D.J. (1999) HMG-1 stimulates estrogen response element binding by estrogen receptor from stably transfected HeLa cells.	bind
36241	2	8650	7	NULL	NULL	0	NULL	HMG-1	NULL		stimulates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_485	11452016	74       Zhang,C.C., Krieg,S. and Shapiro,D.J. (1999) HMG-1 stimulates estrogen response element binding by estrogen receptor from stably transfected HeLa cells.	bind
37288	1	8651	5	13	NULL	NULL	NULL	74-5H7	GP		bind					L1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_7_1223_s_157	12082080	74-5H7 binding to L1 is dynamically regulated by cell - cell contact, L1 - L1 homophilic interactions, and L1 cross-linking   The results of immunocytochemical studies reported in  Fig. 1 suggested that 74-5H7-IR might be induced by cell - cell contact.	bind
37289	2	8651	5	13	NULL	NULL	NULL	statement 1	Process		regulated by		dynamically			cell - cell contact	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_7_1223_s_157	12082080	74-5H7 binding to L1 is dynamically regulated by cell - cell contact, L1 - L1 homophilic interactions, and L1 cross-linking   The results of immunocytochemical studies reported in  Fig. 1 suggested that 74-5H7-IR might be induced by cell - cell contact.	bind
37290	3	8651	5	13	NULL	NULL	NULL	L1	GP		interacts with		homophilically			L1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_7_1223_s_157	12082080	74-5H7 binding to L1 is dynamically regulated by cell - cell contact, L1 - L1 homophilic interactions, and L1 cross-linking   The results of immunocytochemical studies reported in  Fig. 1 suggested that 74-5H7-IR might be induced by cell - cell contact.	bind
37291	4	8651	5	13	NULL	NULL	NULL	statement 1	Process		regulated by		dynamically			L1 	GP	cross-linking of 			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_7_1223_s_157	12082080	74-5H7 binding to L1 is dynamically regulated by cell - cell contact, L1 - L1 homophilic interactions, and L1 cross-linking   The results of immunocytochemical studies reported in  Fig. 1 suggested that 74-5H7-IR might be induced by cell - cell contact.	bind
37292	5	8651	5	13	NULL	NULL	NULL	74-5H7-IR	GP		induced by		might be			cell - cell contact	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_7_1223_s_157	12082080	74-5H7 binding to L1 is dynamically regulated by cell - cell contact, L1 - L1 homophilic interactions, and L1 cross-linking   The results of immunocytochemical studies reported in  Fig. 1 suggested that 74-5H7-IR might be induced by cell - cell contact.	bind
56233	6	8651	5	13	NULL	NULL	NULL	statement 1	Process		is regulated by		dynamically			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_7_1223_s_157	12082080	74-5H7 binding to L1 is dynamically regulated by cell - cell contact, L1 - L1 homophilic interactions, and L1 cross-linking   The results of immunocytochemical studies reported in  Fig. 1 suggested that 74-5H7-IR might be induced by cell - cell contact.	bind
36242	1	8651	7	NULL	NULL	0	NULL	74-5H7	NULL		bind	NULL				L1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_7_1223_s_157	12082080	74-5H7 binding to L1 is dynamically regulated by cell - cell contact, L1 - L1 homophilic interactions, and L1 cross-linking   The results of immunocytochemical studies reported in  Fig. 1 suggested that 74-5H7-IR might be induced by cell - cell contact.	bind
36243	2	8651	7	NULL	NULL	0	NULL	cell - cell contact	NULL		regulates	NULL	dynamically			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_157_7_1223_s_157	12082080	74-5H7 binding to L1 is dynamically regulated by cell - cell contact, L1 - L1 homophilic interactions, and L1 cross-linking   The results of immunocytochemical studies reported in  Fig. 1 suggested that 74-5H7-IR might be induced by cell - cell contact.	bind
36244	3	8651	7	NULL	NULL	0	NULL	L1	NULL		interacts with	NULL	homophilic			L1	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_157_7_1223_s_157	12082080	74-5H7 binding to L1 is dynamically regulated by cell - cell contact, L1 - L1 homophilic interactions, and L1 cross-linking   The results of immunocytochemical studies reported in  Fig. 1 suggested that 74-5H7-IR might be induced by cell - cell contact.	bind
36245	4	8651	7	NULL	NULL	0	NULL	statement 3	NULL		regulates	NULL	dynamically			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_157_7_1223_s_157	12082080	74-5H7 binding to L1 is dynamically regulated by cell - cell contact, L1 - L1 homophilic interactions, and L1 cross-linking   The results of immunocytochemical studies reported in  Fig. 1 suggested that 74-5H7-IR might be induced by cell - cell contact.	bind
36246	5	8651	7	NULL	NULL	0	NULL	L1	NULL	crosslinking of	regulates	NULL	dynamically			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_157_7_1223_s_157	12082080	74-5H7 binding to L1 is dynamically regulated by cell - cell contact, L1 - L1 homophilic interactions, and L1 cross-linking   The results of immunocytochemical studies reported in  Fig. 1 suggested that 74-5H7-IR might be induced by cell - cell contact.	bind
36247	6	8651	7	NULL	NULL	0	NULL	cell - cell contact	NULL		induce	NULL	may			74-5H7-IR	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_157_7_1223_s_157	12082080	74-5H7 binding to L1 is dynamically regulated by cell - cell contact, L1 - L1 homophilic interactions, and L1 cross-linking   The results of immunocytochemical studies reported in  Fig. 1 suggested that 74-5H7-IR might be induced by cell - cell contact.	bind
37293	1	8652	5	13	NULL	NULL	NULL	74-5H7	GP		bind		strongly			L1	GP				NULL	extract lacking inhibitors	NULL	NULL	NULL	NULL	gw60_cellbiol_157_7_1223_s_143	12082080	74-5H7 binds much more strongly to L1 in the extract lacking the inhibitors.	bind
36248	1	8652	7	10	NULL	0	NULL	74-5H7	NULL		bind	NULL	strongly			L1	NULL				NULL	extract lacking the inhibitors	NULL	NULL	NULL	NULL	gw60_cellbiol_157_7_1223_s_143	12082080	74-5H7 binds much more strongly to L1 in the extract lacking the inhibitors.	bind
37294	1	8653	5	13	NULL	NULL	NULL	HMG-I	GP		is a type of					DNA-bending protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_489	11452016	75       Onate,S., Prendergast,P., Wagner,J.P., Nissen,M., Reeves,R., Pettijohn,D.E. and Edwards,D.P. (1994) The DNA-bending protein HMG-I enhances progesterone receptor binding to its target DNA sequences.	bind
37295	2	8653	5	13	NULL	NULL	NULL	progesterone receptor	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_489	11452016	75       Onate,S., Prendergast,P., Wagner,J.P., Nissen,M., Reeves,R., Pettijohn,D.E. and Edwards,D.P. (1994) The DNA-bending protein HMG-I enhances progesterone receptor binding to its target DNA sequences.	bind
37296	3	8653	5	13	NULL	NULL	NULL	HMG-1	GP		enhance					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_489	11452016	75       Onate,S., Prendergast,P., Wagner,J.P., Nissen,M., Reeves,R., Pettijohn,D.E. and Edwards,D.P. (1994) The DNA-bending protein HMG-I enhances progesterone receptor binding to its target DNA sequences.	bind
36250	1	8653	7	NULL	NULL	0	NULL	progesterone receptor	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_489	11452016	75       Onate,S., Prendergast,P., Wagner,J.P., Nissen,M., Reeves,R., Pettijohn,D.E. and Edwards,D.P. (1994) The DNA-bending protein HMG-I enhances progesterone receptor binding to its target DNA sequences.	bind
36251	2	8653	7	NULL	NULL	0	NULL	HMG-I	NULL		enhance	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_489	11452016	75       Onate,S., Prendergast,P., Wagner,J.P., Nissen,M., Reeves,R., Pettijohn,D.E. and Edwards,D.P. (1994) The DNA-bending protein HMG-I enhances progesterone receptor binding to its target DNA sequences.	bind
36252	3	8653	7	NULL	NULL	0	NULL	HMG-1	NULL		is a type of	NULL				DNA-bending protein	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_489	11452016	75       Onate,S., Prendergast,P., Wagner,J.P., Nissen,M., Reeves,R., Pettijohn,D.E. and Edwards,D.P. (1994) The DNA-bending protein HMG-I enhances progesterone receptor binding to its target DNA sequences.	bind
37297	1	8654	5	13	NULL	NULL	NULL	talin	GP		does not bind					beta3	GP	phosphorylated;; cytoplasmic	 tyrosine		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_11_1971_s_129	12947018	75 - 77   Neither talin nor Syk binds to beta3 when both cytoplasmic tyrosine residues are phosphorylated, 70,78  whereas nonmuscle myosin A only binds to beta3 when both cytoplasmic tyrosine residues are phosphorylated.	bind
37298	2	8654	5	13	NULL	NULL	NULL	Syk	GP		does not bind					beta3	GP	phosphorylated;; cytoplasmic	tyrosine		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_11_1971_s_129	12947018	75 - 77   Neither talin nor Syk binds to beta3 when both cytoplasmic tyrosine residues are phosphorylated, 70,78  whereas nonmuscle myosin A only binds to beta3 when both cytoplasmic tyrosine residues are phosphorylated.	bind
37299	3	8654	5	13	NULL	NULL	NULL	myosin A	GP	nonmuscle	bind					beta3	GP	phosphorylated;; cytoplasmic	tyrosine		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_11_1971_s_129	12947018	75 - 77   Neither talin nor Syk binds to beta3 when both cytoplasmic tyrosine residues are phosphorylated, 70,78  whereas nonmuscle myosin A only binds to beta3 when both cytoplasmic tyrosine residues are phosphorylated.	bind
36253	1	8654	7	10	NULL	0	NULL	talin	NULL		does not bind	NULL				beta3	NULL	phosphorylated;; cytoplasmic	tyrosine		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_11_1971_s_129	12947018	75 - 77   Neither talin nor Syk binds to beta3 when both cytoplasmic tyrosine residues are phosphorylated, 70,78  whereas nonmuscle myosin A only binds to beta3 when both cytoplasmic tyrosine residues are phosphorylated.	bind
36254	2	8654	7	10	NULL	0	NULL	Syk	NULL		does not bind	NULL				beta3	NULL	phosphorylated;; cytoplasmic	tyrosine		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_11_1971_s_129	12947018	75 - 77   Neither talin nor Syk binds to beta3 when both cytoplasmic tyrosine residues are phosphorylated, 70,78  whereas nonmuscle myosin A only binds to beta3 when both cytoplasmic tyrosine residues are phosphorylated.	bind
36256	5	8654	7	10	NULL	0	NULL	myosin A		nonmuscle 	binds					beta3		phosphorylated;; cytoplasmic	tyrosine		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_11_1971_s_129	12947018	75 - 77   Neither talin nor Syk binds to beta3 when both cytoplasmic tyrosine residues are phosphorylated, 70,78  whereas nonmuscle myosin A only binds to beta3 when both cytoplasmic tyrosine residues are phosphorylated.	bind
37300	1	8655	5	13	NULL	NULL	NULL	tropomyosin	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_6_580_s_170	9742053	75 89 90 91  Two of them, A63V and K70T, are located in exon 2b within the consensus pattern of sequence repeats of alpha-TM and could alter tropomyosin binding to actin.	bind
37301	2	8655	5	13	NULL	NULL	NULL	alpha-TM	GP		located in			A63V;;K70T		alpha-TM	GP			exon 2b	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_6_580_s_170	9742053	75 89 90 91  Two of them, A63V and K70T, are located in exon 2b within the consensus pattern of sequence repeats of alpha-TM and could alter tropomyosin binding to actin.	bind
37302	3	8655	5	13	NULL	NULL	NULL	statement 2	Process		alters					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_83_6_580_s_170	9742053	75 89 90 91  Two of them, A63V and K70T, are located in exon 2b within the consensus pattern of sequence repeats of alpha-TM and could alter tropomyosin binding to actin.	bind
36259	1	8655	7	NULL	NULL	0	NULL	tropomyosin 	NULL		bind	NULL				actin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_6_580_s_170	9742053	75 89 90 91  Two of them, A63V and K70T, are located in exon 2b within the consensus pattern of sequence repeats of alpha-TM and could alter tropomyosin binding to actin.	bind
36260	2	8655	7	NULL	NULL	0	NULL		NULL		is located in	NULL		 A63V		alpha-TM	NULL			exon 2b	NULL		0	NULL	NULL	NULL	gw60_circulationres_83_6_580_s_170	9742053	75 89 90 91  Two of them, A63V and K70T, are located in exon 2b within the consensus pattern of sequence repeats of alpha-TM and could alter tropomyosin binding to actin.	bind
36261	3	8655	7	NULL	NULL	0	NULL		NULL		is located in	NULL		 K70T		alpha-TM	NULL			exon 2b	NULL		0	NULL	NULL	NULL	gw60_circulationres_83_6_580_s_170	9742053	75 89 90 91  Two of them, A63V and K70T, are located in exon 2b within the consensus pattern of sequence repeats of alpha-TM and could alter tropomyosin binding to actin.	bind
36262	4	8655	7	NULL	NULL	0	NULL		NULL		alters	NULL		A63V		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_6_580_s_170	9742053	75 89 90 91  Two of them, A63V and K70T, are located in exon 2b within the consensus pattern of sequence repeats of alpha-TM and could alter tropomyosin binding to actin.	bind
36263	5	8655	7	NULL	NULL	0	NULL		NULL		alters	NULL		K70T		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_6_580_s_170	9742053	75 89 90 91  Two of them, A63V and K70T, are located in exon 2b within the consensus pattern of sequence repeats of alpha-TM and could alter tropomyosin binding to actin.	bind
37717	1	8656	5	13	NULL	NULL	NULL	alpha2beta1	GP		bind					collagens	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_1_35_s_196	10617582	75 mug/ml or 7 muM;  Mr 11,112 (Fig.  8 A), and of alpha2beta1 and alpha2 A-domain binding to these collagens (IC50 ~30 mug/ml or 3 muM; Fig.  8,  B-D), confirming the identity of GFOGER as an alpha2beta1 integrin recognition site and establishing the crucial importance of this sequence as a platelet alpha2beta1-binding locus in collagens I and IV.	bind
37718	2	8656	5	13	NULL	NULL	NULL	alpha2	GP		bind			A domain		collagens	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_1_35_s_196	10617582	75 mug/ml or 7 muM;  Mr 11,112 (Fig.  8 A), and of alpha2beta1 and alpha2 A-domain binding to these collagens (IC50 ~30 mug/ml or 3 muM; Fig.  8,  B-D), confirming the identity of GFOGER as an alpha2beta1 integrin recognition site and establishing the crucial importance of this sequence as a platelet alpha2beta1-binding locus in collagens I and IV.	bind
37719	3	8656	5	13	NULL	NULL	NULL	GFOGER	GP		recognizes					alpha2beta1 integrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_1_35_s_196	10617582	75 mug/ml or 7 muM;  Mr 11,112 (Fig.  8 A), and of alpha2beta1 and alpha2 A-domain binding to these collagens (IC50 ~30 mug/ml or 3 muM; Fig.  8,  B-D), confirming the identity of GFOGER as an alpha2beta1 integrin recognition site and establishing the crucial importance of this sequence as a platelet alpha2beta1-binding locus in collagens I and IV.	bind
37720	4	8656	5	13	NULL	NULL	NULL				acts as			GFOGER		collagen I	GP	platelet 	alpha2beta1-binding locus		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_1_35_s_196	10617582	75 mug/ml or 7 muM;  Mr 11,112 (Fig.  8 A), and of alpha2beta1 and alpha2 A-domain binding to these collagens (IC50 ~30 mug/ml or 3 muM; Fig.  8,  B-D), confirming the identity of GFOGER as an alpha2beta1 integrin recognition site and establishing the crucial importance of this sequence as a platelet alpha2beta1-binding locus in collagens I and IV.	bind
37721	5	8656	5	13	NULL	NULL	NULL				acts as			GFOGER		collagen IV	GP	platelet	alpha2beta1-binding locus		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_1_35_s_196	10617582	75 mug/ml or 7 muM;  Mr 11,112 (Fig.  8 A), and of alpha2beta1 and alpha2 A-domain binding to these collagens (IC50 ~30 mug/ml or 3 muM; Fig.  8,  B-D), confirming the identity of GFOGER as an alpha2beta1 integrin recognition site and establishing the crucial importance of this sequence as a platelet alpha2beta1-binding locus in collagens I and IV.	bind
36264	1	8656	7	10	NULL	0	NULL	alpha2beta1			bind					collagen					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_1_35_s_196	10617582	75 mug/ml or 7 muM;  Mr 11,112 (Fig.  8 A), and of alpha2beta1 and alpha2 A-domain binding to these collagens (IC50 ~30 mug/ml or 3 muM; Fig.  8,  B-D), confirming the identity of GFOGER as an alpha2beta1 integrin recognition site and establishing the crucial importance of this sequence as a platelet alpha2beta1-binding locus in collagens I and IV.	bind
36265	2	8656	7	NULL	NULL	0	NULL	alpha2	NULL		bind	NULL		A-domain		collagen	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_1_35_s_196	10617582	75 mug/ml or 7 muM;  Mr 11,112 (Fig.  8 A), and of alpha2beta1 and alpha2 A-domain binding to these collagens (IC50 ~30 mug/ml or 3 muM; Fig.  8,  B-D), confirming the identity of GFOGER as an alpha2beta1 integrin recognition site and establishing the crucial importance of this sequence as a platelet alpha2beta1-binding locus in collagens I and IV.	bind
36266	3	8656	7	NULL	NULL	0	NULL		NULL		recognizes	NULL		GFOGER 		alpha2beta1 integrin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_1_35_s_196	10617582	75 mug/ml or 7 muM;  Mr 11,112 (Fig.  8 A), and of alpha2beta1 and alpha2 A-domain binding to these collagens (IC50 ~30 mug/ml or 3 muM; Fig.  8,  B-D), confirming the identity of GFOGER as an alpha2beta1 integrin recognition site and establishing the crucial importance of this sequence as a platelet alpha2beta1-binding locus in collagens I and IV.	bind
36267	4	8656	7	10	NULL	0	NULL	GFOGER			acts as					collagen I		platelet	alpha2beta1 binding locus		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_1_35_s_196	10617582	75 mug/ml or 7 muM;  Mr 11,112 (Fig.  8 A), and of alpha2beta1 and alpha2 A-domain binding to these collagens (IC50 ~30 mug/ml or 3 muM; Fig.  8,  B-D), confirming the identity of GFOGER as an alpha2beta1 integrin recognition site and establishing the crucial importance of this sequence as a platelet alpha2beta1-binding locus in collagens I and IV.	bind
36268	5	8656	7	10	NULL	0	NULL	GFOGER			acts as					collagen IV		platelet	alpha2beta1 binding locus		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_1_35_s_196	10617582	75 mug/ml or 7 muM;  Mr 11,112 (Fig.  8 A), and of alpha2beta1 and alpha2 A-domain binding to these collagens (IC50 ~30 mug/ml or 3 muM; Fig.  8,  B-D), confirming the identity of GFOGER as an alpha2beta1 integrin recognition site and establishing the crucial importance of this sequence as a platelet alpha2beta1-binding locus in collagens I and IV.	bind
37303	1	8657	5	13	NULL	NULL	NULL	p53	GP		bind		sequence specifically			DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_20_4114_s_620	11600700	77       Gu,W. and Roeder,R.G. (1997) Activation of p53 sequence-specific DNA binding by acetylation of the p53 C-terminal domain.	bind
37304	2	8657	5	13	NULL	NULL	NULL	p53	GP	acetylation of	activates			C-terminal domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_20_4114_s_620	11600700	77       Gu,W. and Roeder,R.G. (1997) Activation of p53 sequence-specific DNA binding by acetylation of the p53 C-terminal domain.	bind
36271	1	8657	7	NULL	NULL	0	NULL	 p53	NULL		bind	NULL	sequence-specific			DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_20_4114_s_620	11600700	77       Gu,W. and Roeder,R.G. (1997) Activation of p53 sequence-specific DNA binding by acetylation of the p53 C-terminal domain.	bind
36272	2	8657	7	NULL	NULL	0	NULL	p53	NULL	acetylation of	activates	NULL		C-terminal domain		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_20_4114_s_620	11600700	77       Gu,W. and Roeder,R.G. (1997) Activation of p53 sequence-specific DNA binding by acetylation of the p53 C-terminal domain.	bind
37315	1	8658	5	13	NULL	NULL	NULL	LDL	GP	131 I-cyclohexanedione treated	does not bind					receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3542_s_302	9437204	77  111 113  We also found that tracer  131 I-cyclohexanedione treated LDL that does not bind to receptors gave a relatively constant low daily U/P ratio 111 (Fig 5B  ), evidence that the early rapid clearance of LDL from plasma was due to the action of LDL receptors.	bind
37316	2	8658	5	13	NULL	NULL	NULL	LDL	GP		is cleared from		early;;rapidly			plasma	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3542_s_302	9437204	77  111 113  We also found that tracer  131 I-cyclohexanedione treated LDL that does not bind to receptors gave a relatively constant low daily U/P ratio 111 (Fig 5B  ), evidence that the early rapid clearance of LDL from plasma was due to the action of LDL receptors.	bind
36273	1	8658	7	NULL	NULL	0	NULL	LDL receptor	NULL		clears	NULL				LDL	NULL				NULL	plasma	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3542_s_302	9437204	77  111 113  We also found that tracer  131 I-cyclohexanedione treated LDL that does not bind to receptors gave a relatively constant low daily U/P ratio 111 (Fig 5B  ), evidence that the early rapid clearance of LDL from plasma was due to the action of LDL receptors.	bind
36274	2	8658	7	NULL	NULL	0	NULL	 LDL	NULL	131 I-cyclohexanedione treated	does not bind	NULL				receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3542_s_302	9437204	77  111 113  We also found that tracer  131 I-cyclohexanedione treated LDL that does not bind to receptors gave a relatively constant low daily U/P ratio 111 (Fig 5B  ), evidence that the early rapid clearance of LDL from plasma was due to the action of LDL receptors.	bind
37318	1	8659	5	13	NULL	NULL	NULL	transcription factors	GP		bind					DNA	NucleicAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulationres_85_8_753_s_195	10521248	78 111  112 113  Many of the reported studies demonstrate changes in the in vitro DNA binding activity of transcription factors in response to oxidants or reductants.	bind
37319	2	8659	5	13	NULL	NULL	NULL	oxidants	Chemical		changes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_8_753_s_195	10521248	78 111  112 113  Many of the reported studies demonstrate changes in the in vitro DNA binding activity of transcription factors in response to oxidants or reductants.	bind
37320	3	8659	5	13	NULL	NULL	NULL	reductants	Chemical		changes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_8_753_s_195	10521248	78 111  112 113  Many of the reported studies demonstrate changes in the in vitro DNA binding activity of transcription factors in response to oxidants or reductants.	bind
36275	1	8659	7	NULL	NULL	0	NULL	transcription factor	NULL		bind	NULL				DNA	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulationres_85_8_753_s_195	10521248	78 111  112 113  Many of the reported studies demonstrate changes in the in vitro DNA binding activity of transcription factors in response to oxidants or reductants.	bind
36276	2	8659	7	NULL	NULL	0	NULL	oxidants	NULL		change	NULL				statement 1	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulationres_85_8_753_s_195	10521248	78 111  112 113  Many of the reported studies demonstrate changes in the in vitro DNA binding activity of transcription factors in response to oxidants or reductants.	bind
36277	3	8659	7	NULL	NULL	0	NULL	reductants	NULL		change	NULL				statement 2	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_circulationres_85_8_753_s_195	10521248	78 111  112 113  Many of the reported studies demonstrate changes in the in vitro DNA binding activity of transcription factors in response to oxidants or reductants.	bind
37321	1	8660	5	13	NULL	NULL	NULL	7E cell line	Cell		is a type of					IgG2b isotype	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_10_2251_s_47	8636404	7E cell line is of the IgG2b isotype, and binds both PC and dsDNA by ELISA.	bind
37322	2	8660	5	13	NULL	NULL	NULL	7E cell line	Cell		bind					PC	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_10_2251_s_47	8636404	7E cell line is of the IgG2b isotype, and binds both PC and dsDNA by ELISA.	bind
37323	3	8660	5	13	NULL	NULL	NULL	7E cell line	Cell		bind					dsDNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_10_2251_s_47	8636404	7E cell line is of the IgG2b isotype, and binds both PC and dsDNA by ELISA.	bind
36278	1	8660	7	NULL	NULL	0	NULL	PC	NULL		bind	NULL				7E cell line	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_97_10_2251_s_47	8636404	7E cell line is of the IgG2b isotype, and binds both PC and dsDNA by ELISA.	bind
36279	2	8660	7	NULL	NULL	0	NULL	dsDNA	NULL		bind	NULL				7E cell line	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_97_10_2251_s_47	8636404	7E cell line is of the IgG2b isotype, and binds both PC and dsDNA by ELISA.	bind
36280	3	8660	7	NULL	NULL	0	NULL	7E cell line	NULL		is a type of	NULL				IgG2b isotype	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_97_10_2251_s_47	8636404	7E cell line is of the IgG2b isotype, and binds both PC and dsDNA by ELISA.	bind
37324	1	8661	5	13	NULL	NULL	NULL	transducin	GP		bind					rhodopsin membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_49_51203_s_67	15351781	7PP and arrestin inhibit light- and GTP-dependent binding of transducin to rhodopsin  membranes.	bind
37325	2	8661	5	13	NULL	NULL	NULL	statement 1	Process		is dependent on					light					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_49_51203_s_67	15351781	7PP and arrestin inhibit light- and GTP-dependent binding of transducin to rhodopsin  membranes.	bind
37326	3	8661	5	13	NULL	NULL	NULL	statement 1	Process		is dependent on					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_49_51203_s_67	15351781	7PP and arrestin inhibit light- and GTP-dependent binding of transducin to rhodopsin  membranes.	bind
37327	4	8661	5	13	NULL	NULL	NULL	7PP	GP		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_49_51203_s_67	15351781	7PP and arrestin inhibit light- and GTP-dependent binding of transducin to rhodopsin  membranes.	bind
37328	5	8661	5	13	NULL	NULL	NULL	7PP	GP		inhibit					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_49_51203_s_67	15351781	7PP and arrestin inhibit light- and GTP-dependent binding of transducin to rhodopsin  membranes.	bind
37329	6	8661	5	13	NULL	NULL	NULL	arrestin	GP		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_49_51203_s_67	15351781	7PP and arrestin inhibit light- and GTP-dependent binding of transducin to rhodopsin  membranes.	bind
37330	7	8661	5	13	NULL	NULL	NULL	arrestin	GP		inhibit					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_49_51203_s_67	15351781	7PP and arrestin inhibit light- and GTP-dependent binding of transducin to rhodopsin  membranes.	bind
36281	1	8661	7	NULL	NULL	0	NULL	transducin	NULL		bind	NULL				rhodopsin membrane	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_49_51203_s_67	15351781	7PP and arrestin inhibit light- and GTP-dependent binding of transducin to rhodopsin  membranes.	bind
36282	2	8661	7	NULL	NULL	0	NULL	statement 1	NULL		depends on	NULL				GTP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_49_51203_s_67	15351781	7PP and arrestin inhibit light- and GTP-dependent binding of transducin to rhodopsin  membranes.	bind
36283	3	8661	7	NULL	NULL	0	NULL	statement 1	NULL		depends on	NULL				light	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_49_51203_s_67	15351781	7PP and arrestin inhibit light- and GTP-dependent binding of transducin to rhodopsin  membranes.	bind
36284	4	8661	7	NULL	NULL	0	NULL	7PP	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_49_51203_s_67	15351781	7PP and arrestin inhibit light- and GTP-dependent binding of transducin to rhodopsin  membranes.	bind
36285	5	8661	7	NULL	NULL	0	NULL	7PP	NULL		inhibits	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_49_51203_s_67	15351781	7PP and arrestin inhibit light- and GTP-dependent binding of transducin to rhodopsin  membranes.	bind
36286	6	8661	7	NULL	NULL	0	NULL	arrestin	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_49_51203_s_67	15351781	7PP and arrestin inhibit light- and GTP-dependent binding of transducin to rhodopsin  membranes.	bind
36287	7	8661	7	NULL	NULL	0	NULL	arrestin	NULL		inhibits	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_49_51203_s_67	15351781	7PP and arrestin inhibit light- and GTP-dependent binding of transducin to rhodopsin  membranes.	bind
37331	1	8662	5	13	NULL	NULL	NULL	nod factor	GP		bind					lectin	GP				NULL	legume roots	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_17_3459_s_256	11522814	8       Etzler,M.E., Kalsi,G., Ewing,N.N., Roberts,N.J., Day,R.B. and Murphy,J.B. (1999) A nod factor binding lectin with apyrase activity from legume roots.	bind
37332	2	8662	5	13	NULL	NULL	NULL	lectin	GP		contains					apyrase activity	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_17_3459_s_256	11522814	8       Etzler,M.E., Kalsi,G., Ewing,N.N., Roberts,N.J., Day,R.B. and Murphy,J.B. (1999) A nod factor binding lectin with apyrase activity from legume roots.	bind
36288	1	8662	7	NULL	NULL	0	NULL	nod factor	NULL		bind	NULL				lectin	NULL				NULL	legume roots	0	NULL	NULL	NULL	gw60_nucleicacidsres_29_17_3459_s_256	11522814	8       Etzler,M.E., Kalsi,G., Ewing,N.N., Roberts,N.J., Day,R.B. and Murphy,J.B. (1999) A nod factor binding lectin with apyrase activity from legume roots.	bind
36289	2	8662	7	NULL	NULL	0	NULL	lectin	NULL		contains	NULL				apyrase activity	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_17_3459_s_256	11522814	8       Etzler,M.E., Kalsi,G., Ewing,N.N., Roberts,N.J., Day,R.B. and Murphy,J.B. (1999) A nod factor binding lectin with apyrase activity from legume roots.	bind
37333	1	8663	5	13	NULL	NULL	NULL	nuclear cap binding complex	GP	yeast	interact with					eIF4G	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_5_1080_s_254	11222757	8       Fortes,P., Inada,T., Preiss,T., Hentze,M.W., Mattaj,I.W. and Sachs,A.B. (2000) The yeast nuclear cap binding complex can interact with translation factor eIF4G and mediate translation initiation.	bind
37334	2	8663	5	13	NULL	NULL	NULL	eIF4G	GP		is a type of					translation factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_5_1080_s_254	11222757	8       Fortes,P., Inada,T., Preiss,T., Hentze,M.W., Mattaj,I.W. and Sachs,A.B. (2000) The yeast nuclear cap binding complex can interact with translation factor eIF4G and mediate translation initiation.	bind
37335	3	8663	5	13	NULL	NULL	NULL	statement 1	Process		mediate					translation	Process	initiation of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_5_1080_s_254	11222757	8       Fortes,P., Inada,T., Preiss,T., Hentze,M.W., Mattaj,I.W. and Sachs,A.B. (2000) The yeast nuclear cap binding complex can interact with translation factor eIF4G and mediate translation initiation.	bind
36290	1	8663	7	NULL	NULL	0	NULL	nuclear cap binding complex	NULL	yeast	interacts with	NULL				eIF4G	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_5_1080_s_254	11222757	8       Fortes,P., Inada,T., Preiss,T., Hentze,M.W., Mattaj,I.W. and Sachs,A.B. (2000) The yeast nuclear cap binding complex can interact with translation factor eIF4G and mediate translation initiation.	bind
36291	2	8663	7	NULL	NULL	0	NULL	statement 1	NULL		mediate	NULL				translation	NULL	initiation of			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_5_1080_s_254	11222757	8       Fortes,P., Inada,T., Preiss,T., Hentze,M.W., Mattaj,I.W. and Sachs,A.B. (2000) The yeast nuclear cap binding complex can interact with translation factor eIF4G and mediate translation initiation.	bind
36292	3	8663	7	NULL	NULL	0	NULL	eIF4G	NULL		is a type of	NULL				translation factor	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_5_1080_s_254	11222757	8       Fortes,P., Inada,T., Preiss,T., Hentze,M.W., Mattaj,I.W. and Sachs,A.B. (2000) The yeast nuclear cap binding complex can interact with translation factor eIF4G and mediate translation initiation.	bind
37336	1	8664	5	13	NULL	NULL	NULL	retinoblastoma protein	GP		bind					E2F residues	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_15_3131_s_207	11470869	8       Hagemeier,C., Cook,A. and Kouzarides,T. (1993) The retinoblastoma protein binds E2F residues required for activation  in vivo and TBP binding  in vitro.	bind
37337	2	8664	5	13	NULL	NULL	NULL	E2F residues	GP		is required for					TBP	GP	binding of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_15_3131_s_207	11470869	8       Hagemeier,C., Cook,A. and Kouzarides,T. (1993) The retinoblastoma protein binds E2F residues required for activation  in vivo and TBP binding  in vitro.	bind
36293	1	8664	7	NULL	NULL	0	NULL	 retinoblastoma protein	NULL		binds	NULL				E2F residues	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_15_3131_s_207	11470869	8       Hagemeier,C., Cook,A. and Kouzarides,T. (1993) The retinoblastoma protein binds E2F residues required for activation  in vivo and TBP binding  in vitro.	bind
36295	2	8664	7	10	NULL	0	NULL	statement 1			is required for					TBP		binding of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_15_3131_s_207	11470869	8       Hagemeier,C., Cook,A. and Kouzarides,T. (1993) The retinoblastoma protein binds E2F residues required for activation  in vivo and TBP binding  in vitro.	bind
37338	1	8665	5	13	NULL	NULL	NULL	XPA	GP		bind					RPA	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_4948_s_197	11812824	8       Matsuda,T., Saijo,M., Kuraoka,I., Kobayashi,T., Nakatsu,Y., Nagai,A., Enjoji,T., Masutani,C., Sugasawa,K., Hanaoka,F., Yasui,A. and Tanaka,K. (1995) DNA repair protein XPA binds replication protein A (RPA).	bind
37339	2	8665	5	13	NULL	NULL	NULL	XPA	GP		is a type of					DNA repair protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_4948_s_197	11812824	8       Matsuda,T., Saijo,M., Kuraoka,I., Kobayashi,T., Nakatsu,Y., Nagai,A., Enjoji,T., Masutani,C., Sugasawa,K., Hanaoka,F., Yasui,A. and Tanaka,K. (1995) DNA repair protein XPA binds replication protein A (RPA).	bind
37340	3	8665	5	13	NULL	NULL	NULL	RPA	GP		is					replication protein A	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_4948_s_197	11812824	8       Matsuda,T., Saijo,M., Kuraoka,I., Kobayashi,T., Nakatsu,Y., Nagai,A., Enjoji,T., Masutani,C., Sugasawa,K., Hanaoka,F., Yasui,A. and Tanaka,K. (1995) DNA repair protein XPA binds replication protein A (RPA).	bind
36296	1	8665	7	NULL	NULL	0	NULL	XPA	NULL		binds	NULL				RPA	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_4948_s_197	11812824	8       Matsuda,T., Saijo,M., Kuraoka,I., Kobayashi,T., Nakatsu,Y., Nagai,A., Enjoji,T., Masutani,C., Sugasawa,K., Hanaoka,F., Yasui,A. and Tanaka,K. (1995) DNA repair protein XPA binds replication protein A (RPA).	bind
36297	2	8665	7	NULL	NULL	0	NULL	XPA	NULL		is a type of	NULL				DNA repair protein	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_4948_s_197	11812824	8       Matsuda,T., Saijo,M., Kuraoka,I., Kobayashi,T., Nakatsu,Y., Nagai,A., Enjoji,T., Masutani,C., Sugasawa,K., Hanaoka,F., Yasui,A. and Tanaka,K. (1995) DNA repair protein XPA binds replication protein A (RPA).	bind
36298	3	8665	7	10	NULL	0	NULL	RPA			is					replication protein A					NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_24_4948_s_197	11812824	8       Matsuda,T., Saijo,M., Kuraoka,I., Kobayashi,T., Nakatsu,Y., Nagai,A., Enjoji,T., Masutani,C., Sugasawa,K., Hanaoka,F., Yasui,A. and Tanaka,K. (1995) DNA repair protein XPA binds replication protein A (RPA).	bind
37341	1	8667	5	13	NULL	NULL	NULL	heparin	Chemical		associate with					antithrombin III	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_163	10510057	8  9 10 11  Besides the anticoagulative effects of heparin mediated by its association with antithrombin III, the described blockade of factor X binding to Mac-1 may participate in the anticoagulative properties of heparin.	bind
37342	2	8667	5	13	NULL	NULL	NULL	heparin	Chemical	anticoagulative effects of	is mediated by					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_163	10510057	8  9 10 11  Besides the anticoagulative effects of heparin mediated by its association with antithrombin III, the described blockade of factor X binding to Mac-1 may participate in the anticoagulative properties of heparin.	bind
37343	3	8667	5	13	NULL	NULL	NULL	factor X	GP		bind					Mac-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_163	10510057	8  9 10 11  Besides the anticoagulative effects of heparin mediated by its association with antithrombin III, the described blockade of factor X binding to Mac-1 may participate in the anticoagulative properties of heparin.	bind
37344	4	8667	5	13	NULL	NULL	NULL	statement 3	Process	blockade of	participate in					heparin	Chemical	anticoagulative properties of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_163	10510057	8  9 10 11  Besides the anticoagulative effects of heparin mediated by its association with antithrombin III, the described blockade of factor X binding to Mac-1 may participate in the anticoagulative properties of heparin.	bind
36610	1	8667	7	NULL	NULL	0	NULL	heparin	NULL		associate with	NULL				antithrombin III	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_163	10510057	8  9 10 11  Besides the anticoagulative effects of heparin mediated by its association with antithrombin III, the described blockade of factor X binding to Mac-1 may participate in the anticoagulative properties of heparin.	bind
36612	2	8667	7	NULL	NULL	0	NULL	factor X	NULL		bind	NULL				Mac-1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_163	10510057	8  9 10 11  Besides the anticoagulative effects of heparin mediated by its association with antithrombin III, the described blockade of factor X binding to Mac-1 may participate in the anticoagulative properties of heparin.	bind
36614	4	8667	7	NULL	NULL	0	NULL	statement 1	NULL		mediates	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_163	10510057	8  9 10 11  Besides the anticoagulative effects of heparin mediated by its association with antithrombin III, the described blockade of factor X binding to Mac-1 may participate in the anticoagulative properties of heparin.	bind
36615	4	8667	7	NULL	NULL	0	NULL	statement 2	NULL	blocking of	participate in	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_163	10510057	8  9 10 11  Besides the anticoagulative effects of heparin mediated by its association with antithrombin III, the described blockade of factor X binding to Mac-1 may participate in the anticoagulative properties of heparin.	bind
46729	3	8667	7	NULL	NULL	0	NULL	heparin	NULL		exhibit	NULL				 anticoagulative properties	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_100_14_1533_s_163	10510057	8  9 10 11  Besides the anticoagulative effects of heparin mediated by its association with antithrombin III, the described blockade of factor X binding to Mac-1 may participate in the anticoagulative properties of heparin.	bind
37345	1	8668	5	13	NULL	NULL	NULL	GSK-3beta	GP		phosphorylate					glycogen synthase	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_5_1597_s_12	11696419	8  Among them are the serine/threonine protein kinase glycogen synthase kinase-3beta (GSK-3beta) 9 and a novel presenilin binding protein named PBP. 10  GSK-3beta was initially purified as an enzyme that phosphorylates and inactivates glycogen synthase, but it was later shown that it has the ability to phosphorylate [[ the neurofibrillary protein tau. 11  PBP ]] was identified by its ability to bind to the large cytoplasmic loop of PS1 in the yeast two-hybrid system.	bind
37346	2	8668	5	13	NULL	NULL	NULL	statement 1	Process		inactivate					glycogen synthase	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_5_1597_s_12	11696419	8  Among them are the serine/threonine protein kinase glycogen synthase kinase-3beta (GSK-3beta) 9 and a novel presenilin binding protein named PBP. 10  GSK-3beta was initially purified as an enzyme that phosphorylates and inactivates glycogen synthase, but it was later shown that it has the ability to phosphorylate [[ the neurofibrillary protein tau. 11  PBP ]] was identified by its ability to bind to the large cytoplasmic loop of PS1 in the yeast two-hybrid system.	bind
37347	3	8668	5	13	NULL	NULL	NULL	GSK-3beta	GP		is					glycogen synthase kinase-3beta	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_5_1597_s_12	11696419	8  Among them are the serine/threonine protein kinase glycogen synthase kinase-3beta (GSK-3beta) 9 and a novel presenilin binding protein named PBP. 10  GSK-3beta was initially purified as an enzyme that phosphorylates and inactivates glycogen synthase, but it was later shown that it has the ability to phosphorylate [[ the neurofibrillary protein tau. 11  PBP ]] was identified by its ability to bind to the large cytoplasmic loop of PS1 in the yeast two-hybrid system.	bind
37348	4	8668	5	13	NULL	NULL	NULL	GSK-3beta	GP		is a type of					serine/threonine protein kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_5_1597_s_12	11696419	8  Among them are the serine/threonine protein kinase glycogen synthase kinase-3beta (GSK-3beta) 9 and a novel presenilin binding protein named PBP. 10  GSK-3beta was initially purified as an enzyme that phosphorylates and inactivates glycogen synthase, but it was later shown that it has the ability to phosphorylate [[ the neurofibrillary protein tau. 11  PBP ]] was identified by its ability to bind to the large cytoplasmic loop of PS1 in the yeast two-hybrid system.	bind
37350	6	8668	5	13	NULL	NULL	NULL	tau	GP		is a type of					neurofibrillary protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_5_1597_s_12	11696419	8  Among them are the serine/threonine protein kinase glycogen synthase kinase-3beta (GSK-3beta) 9 and a novel presenilin binding protein named PBP. 10  GSK-3beta was initially purified as an enzyme that phosphorylates and inactivates glycogen synthase, but it was later shown that it has the ability to phosphorylate [[ the neurofibrillary protein tau. 11  PBP ]] was identified by its ability to bind to the large cytoplasmic loop of PS1 in the yeast two-hybrid system.	bind
37351	7	8668	5	13	NULL	NULL	NULL	PBP	GP		is					presenilin binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_5_1597_s_12	11696419	8  Among them are the serine/threonine protein kinase glycogen synthase kinase-3beta (GSK-3beta) 9 and a novel presenilin binding protein named PBP. 10  GSK-3beta was initially purified as an enzyme that phosphorylates and inactivates glycogen synthase, but it was later shown that it has the ability to phosphorylate [[ the neurofibrillary protein tau. 11  PBP ]] was identified by its ability to bind to the large cytoplasmic loop of PS1 in the yeast two-hybrid system.	bind
37352	8	8668	5	13	NULL	NULL	NULL	PBP	GP		bind					PS1	GP		cytoplasmic loop		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_159_5_1597_s_12	11696419	8  Among them are the serine/threonine protein kinase glycogen synthase kinase-3beta (GSK-3beta) 9 and a novel presenilin binding protein named PBP. 10  GSK-3beta was initially purified as an enzyme that phosphorylates and inactivates glycogen synthase, but it was later shown that it has the ability to phosphorylate [[ the neurofibrillary protein tau. 11  PBP ]] was identified by its ability to bind to the large cytoplasmic loop of PS1 in the yeast two-hybrid system.	bind
36617	1	8668	7	NULL	NULL	0	NULL	GSK-3beta	NULL		phosphorylates	NULL				glycogen synthase	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_5_1597_s_12	11696419	8  Among them are the serine/threonine protein kinase glycogen synthase kinase-3beta (GSK-3beta) 9 and a novel presenilin binding protein named PBP. 10  GSK-3beta was initially purified as an enzyme that phosphorylates and inactivates glycogen synthase, but it was later shown that it has the ability to phosphorylate [[ the neurofibrillary protein tau. 11  PBP ]] was identified by its ability to bind to the large cytoplasmic loop of PS1 in the yeast two-hybrid system.	bind
36619	2	8668	7	NULL	NULL	0	NULL	statement 1	NULL		inactivates	NULL				glycogen synthase	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_5_1597_s_12	11696419	8  Among them are the serine/threonine protein kinase glycogen synthase kinase-3beta (GSK-3beta) 9 and a novel presenilin binding protein named PBP. 10  GSK-3beta was initially purified as an enzyme that phosphorylates and inactivates glycogen synthase, but it was later shown that it has the ability to phosphorylate [[ the neurofibrillary protein tau. 11  PBP ]] was identified by its ability to bind to the large cytoplasmic loop of PS1 in the yeast two-hybrid system.	bind
36621	3	8668	7	NULL	NULL	0	NULL	GSK-3beta	NULL		phosphorylate	NULL				tau	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_5_1597_s_12	11696419	8  Among them are the serine/threonine protein kinase glycogen synthase kinase-3beta (GSK-3beta) 9 and a novel presenilin binding protein named PBP. 10  GSK-3beta was initially purified as an enzyme that phosphorylates and inactivates glycogen synthase, but it was later shown that it has the ability to phosphorylate [[ the neurofibrillary protein tau. 11  PBP ]] was identified by its ability to bind to the large cytoplasmic loop of PS1 in the yeast two-hybrid system.	bind
36624	4	8668	7	NULL	NULL	0	NULL	tau	NULL		is a type of	NULL				neurofibrillary protein	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_5_1597_s_12	11696419	8  Among them are the serine/threonine protein kinase glycogen synthase kinase-3beta (GSK-3beta) 9 and a novel presenilin binding protein named PBP. 10  GSK-3beta was initially purified as an enzyme that phosphorylates and inactivates glycogen synthase, but it was later shown that it has the ability to phosphorylate [[ the neurofibrillary protein tau. 11  PBP ]] was identified by its ability to bind to the large cytoplasmic loop of PS1 in the yeast two-hybrid system.	bind
36626	5	8668	7	NULL	NULL	0	NULL	PBP	NULL		bind	NULL				PS1	NULL		large cytoplasmic loop of 		NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_5_1597_s_12	11696419	8  Among them are the serine/threonine protein kinase glycogen synthase kinase-3beta (GSK-3beta) 9 and a novel presenilin binding protein named PBP. 10  GSK-3beta was initially purified as an enzyme that phosphorylates and inactivates glycogen synthase, but it was later shown that it has the ability to phosphorylate [[ the neurofibrillary protein tau. 11  PBP ]] was identified by its ability to bind to the large cytoplasmic loop of PS1 in the yeast two-hybrid system.	bind
36627	6	8668	7	NULL	NULL	0	NULL	PBP	NULL		is	NULL				presenilin binding protein	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_5_1597_s_12	11696419	8  Among them are the serine/threonine protein kinase glycogen synthase kinase-3beta (GSK-3beta) 9 and a novel presenilin binding protein named PBP. 10  GSK-3beta was initially purified as an enzyme that phosphorylates and inactivates glycogen synthase, but it was later shown that it has the ability to phosphorylate [[ the neurofibrillary protein tau. 11  PBP ]] was identified by its ability to bind to the large cytoplasmic loop of PS1 in the yeast two-hybrid system.	bind
36628	7	8668	7	NULL	NULL	0	NULL	GSK-3beta	NULL		is	NULL				serine/threonine protein kinase glycogen synthase kinase-3beta 	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_159_5_1597_s_12	11696419	8  Among them are the serine/threonine protein kinase glycogen synthase kinase-3beta (GSK-3beta) 9 and a novel presenilin binding protein named PBP. 10  GSK-3beta was initially purified as an enzyme that phosphorylates and inactivates glycogen synthase, but it was later shown that it has the ability to phosphorylate [[ the neurofibrillary protein tau. 11  PBP ]] was identified by its ability to bind to the large cytoplasmic loop of PS1 in the yeast two-hybrid system.	bind
37496	1	8669	5	13	NULL	NULL	NULL	factor VII	GP		inhibit					thrombin	GP	generation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_21_2555_s_124	11382723	8  An alternative explanation might be provided by the hypothesis that factor VIIa is able to overcome the inhibitory effect of factor VII on thrombin generation, thereby displacing factor VII bound to tissue factor, resulting in additional thrombin generation.	bind
37497	2	8669	5	13	NULL	NULL	NULL	factor VIIa	GP		overcomes		potentially			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_21_2555_s_124	11382723	8  An alternative explanation might be provided by the hypothesis that factor VIIa is able to overcome the inhibitory effect of factor VII on thrombin generation, thereby displacing factor VII bound to tissue factor, resulting in additional thrombin generation.	bind
37498	3	8669	5	13	NULL	NULL	NULL	factor VII	GP		bind					tissue factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_21_2555_s_124	11382723	8  An alternative explanation might be provided by the hypothesis that factor VIIa is able to overcome the inhibitory effect of factor VII on thrombin generation, thereby displacing factor VII bound to tissue factor, resulting in additional thrombin generation.	bind
37499	4	8669	5	13	NULL	NULL	NULL	factor VIIa	GP		displaces		potentially			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_21_2555_s_124	11382723	8  An alternative explanation might be provided by the hypothesis that factor VIIa is able to overcome the inhibitory effect of factor VII on thrombin generation, thereby displacing factor VII bound to tissue factor, resulting in additional thrombin generation.	bind
37500	5	8669	5	13	NULL	NULL	NULL	statement 4	Process		results in		potentially			thrombin	GP	generation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_21_2555_s_124	11382723	8  An alternative explanation might be provided by the hypothesis that factor VIIa is able to overcome the inhibitory effect of factor VII on thrombin generation, thereby displacing factor VII bound to tissue factor, resulting in additional thrombin generation.	bind
36629	1	8669	7	NULL	NULL	0	NULL	 factor VII 	NULL		bind	NULL				tissue factor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_21_2555_s_124	11382723	8  An alternative explanation might be provided by the hypothesis that factor VIIa is able to overcome the inhibitory effect of factor VII on thrombin generation, thereby displacing factor VII bound to tissue factor, resulting in additional thrombin generation.	bind
36630	2	8669	7	NULL	NULL	0	NULL	factor VII	NULL		inhibits	NULL				thrombin	NULL	generation of			NULL		0	NULL	NULL	NULL	gw60_circulation_103_21_2555_s_124	11382723	8  An alternative explanation might be provided by the hypothesis that factor VIIa is able to overcome the inhibitory effect of factor VII on thrombin generation, thereby displacing factor VII bound to tissue factor, resulting in additional thrombin generation.	bind
36631	3	8669	7	NULL	NULL	0	NULL	factor VIIa	NULL		displace	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_21_2555_s_124	11382723	8  An alternative explanation might be provided by the hypothesis that factor VIIa is able to overcome the inhibitory effect of factor VII on thrombin generation, thereby displacing factor VII bound to tissue factor, resulting in additional thrombin generation.	bind
36632	4	8669	7	NULL	NULL	0	NULL	factor VIIa	NULL		overcome	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_21_2555_s_124	11382723	8  An alternative explanation might be provided by the hypothesis that factor VIIa is able to overcome the inhibitory effect of factor VII on thrombin generation, thereby displacing factor VII bound to tissue factor, resulting in additional thrombin generation.	bind
36633	5	8669	7	NULL	NULL	0	NULL	statement 4	NULL		results in	NULL				thrombin	NULL	generation of			NULL		0	NULL	NULL	NULL	gw60_circulation_103_21_2555_s_124	11382723	8  An alternative explanation might be provided by the hypothesis that factor VIIa is able to overcome the inhibitory effect of factor VII on thrombin generation, thereby displacing factor VII bound to tissue factor, resulting in additional thrombin generation.	bind
37503	1	8671	5	13	NULL	NULL	NULL	beta2GPI	GP		bind			lysine-rich locus in fifth domain		PLs	Chemical	negatively charged			NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_9_900_s_27	9521339	8  beta2GPI binds negatively charged PLs through a lysine-rich locus in the fifth domain 9  10  and possesses several in vitro properties that define it as an anticoagulant (ie, inhibition of prothrombinase activity, ADP-induced platelet aggregation, or platelet factor IX production).	bind
37504	2	8671	5	13	NULL	NULL	NULL	beta2GPI	GP		is a type of					anticoagulant	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_9_900_s_27	9521339	8  beta2GPI binds negatively charged PLs through a lysine-rich locus in the fifth domain 9  10  and possesses several in vitro properties that define it as an anticoagulant (ie, inhibition of prothrombinase activity, ADP-induced platelet aggregation, or platelet factor IX production).	bind
37505	3	8671	5	13	NULL	NULL	NULL	beta2GPI	GP		inhibit					prothrombinase activity	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_9_900_s_27	9521339	8  beta2GPI binds negatively charged PLs through a lysine-rich locus in the fifth domain 9  10  and possesses several in vitro properties that define it as an anticoagulant (ie, inhibition of prothrombinase activity, ADP-induced platelet aggregation, or platelet factor IX production).	bind
37506	4	8671	5	13	NULL	NULL	NULL	ADP	Chemical		induce					platelet	Cell	aggregation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_9_900_s_27	9521339	8  beta2GPI binds negatively charged PLs through a lysine-rich locus in the fifth domain 9  10  and possesses several in vitro properties that define it as an anticoagulant (ie, inhibition of prothrombinase activity, ADP-induced platelet aggregation, or platelet factor IX production).	bind
37507	5	8671	5	13	NULL	NULL	NULL	beta2GPI	GP		inhibit					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_9_900_s_27	9521339	8  beta2GPI binds negatively charged PLs through a lysine-rich locus in the fifth domain 9  10  and possesses several in vitro properties that define it as an anticoagulant (ie, inhibition of prothrombinase activity, ADP-induced platelet aggregation, or platelet factor IX production).	bind
37508	6	8671	5	13	NULL	NULL	NULL	beta2GPI	GP		inhibit					platelet factor IX	GP	production of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_9_900_s_27	9521339	8  beta2GPI binds negatively charged PLs through a lysine-rich locus in the fifth domain 9  10  and possesses several in vitro properties that define it as an anticoagulant (ie, inhibition of prothrombinase activity, ADP-induced platelet aggregation, or platelet factor IX production).	bind
36635	1	8671	7	10	NULL	0	NULL	beta2GPI 			binds			lysine-rich locus in the fifth domain		PLs		negatively charged			NULL		NULL	NULL	NULL	NULL	gw60_circulation_97_9_900_s_27	9521339	8  beta2GPI binds negatively charged PLs through a lysine-rich locus in the fifth domain 9  10  and possesses several in vitro properties that define it as an anticoagulant (ie, inhibition of prothrombinase activity, ADP-induced platelet aggregation, or platelet factor IX production).	bind
36636	2	8671	7	NULL	NULL	0	NULL	statement 1	NULL		possess	NULL				in vitro properties	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_97_9_900_s_27	9521339	8  beta2GPI binds negatively charged PLs through a lysine-rich locus in the fifth domain 9  10  and possesses several in vitro properties that define it as an anticoagulant (ie, inhibition of prothrombinase activity, ADP-induced platelet aggregation, or platelet factor IX production).	bind
36637	3	8671	7	NULL	NULL	0	NULL	statement 1	NULL		act as an	NULL				anticoagulant	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_97_9_900_s_27	9521339	8  beta2GPI binds negatively charged PLs through a lysine-rich locus in the fifth domain 9  10  and possesses several in vitro properties that define it as an anticoagulant (ie, inhibition of prothrombinase activity, ADP-induced platelet aggregation, or platelet factor IX production).	bind
36638	4	8671	7	NULL	NULL	0	NULL	ADP	NULL		induce	NULL				platelet 	NULL	aggregation of			NULL		0	NULL	NULL	NULL	gw60_circulation_97_9_900_s_27	9521339	8  beta2GPI binds negatively charged PLs through a lysine-rich locus in the fifth domain 9  10  and possesses several in vitro properties that define it as an anticoagulant (ie, inhibition of prothrombinase activity, ADP-induced platelet aggregation, or platelet factor IX production).	bind
36639	5	8671	7	NULL	NULL	0	NULL	statement 1	NULL		inhibits	NULL				prothrombinase activity	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_97_9_900_s_27	9521339	8  beta2GPI binds negatively charged PLs through a lysine-rich locus in the fifth domain 9  10  and possesses several in vitro properties that define it as an anticoagulant (ie, inhibition of prothrombinase activity, ADP-induced platelet aggregation, or platelet factor IX production).	bind
36640	6	8671	7	NULL	NULL	0	NULL	statement 1	NULL		inhibits	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_97_9_900_s_27	9521339	8  beta2GPI binds negatively charged PLs through a lysine-rich locus in the fifth domain 9  10  and possesses several in vitro properties that define it as an anticoagulant (ie, inhibition of prothrombinase activity, ADP-induced platelet aggregation, or platelet factor IX production).	bind
36641	7	8671	7	NULL	NULL	0	NULL	statement 1	NULL		inhibits	NULL				platelet factor IX	NULL	production of			NULL		0	NULL	NULL	NULL	gw60_circulation_97_9_900_s_27	9521339	8  beta2GPI binds negatively charged PLs through a lysine-rich locus in the fifth domain 9  10  and possesses several in vitro properties that define it as an anticoagulant (ie, inhibition of prothrombinase activity, ADP-induced platelet aggregation, or platelet factor IX production).	bind
37509	1	8672	5	13	NULL	NULL	NULL	rabphilin-3A	GP		bind			amino (NH2)-terminal half		Rab3A	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_163_3_889_s_16	12937130	8  Binding of rabphilin-3A to Rab3A occurs via the amino (NH2)-terminal half of rabphilin-3A.	bind
36642	1	8672	7	NULL	NULL	0	NULL	rabphilin-3A	NULL		bind	NULL		amino (NH2)-terminal half of		Rab3A	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_163_3_889_s_16	12937130	8  Binding of rabphilin-3A to Rab3A occurs via the amino (NH2)-terminal half of rabphilin-3A.	bind
37510	1	8673	5	13	NULL	NULL	NULL	apoB-100	GP		bind					LDLR	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_5_826_s_24	9157944	8  Defective apoB-100 has been shown to reduce significantly the binding of apoB-100 to the LDLR, 2 9 10  which results in elevated LDL cholesterol levels in carriers of this mutation.	bind
37511	2	8673	5	13	NULL	NULL	NULL	apoB-100	GP	mutant	reduce		significantly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_5_826_s_24	9157944	8  Defective apoB-100 has been shown to reduce significantly the binding of apoB-100 to the LDLR, 2 9 10  which results in elevated LDL cholesterol levels in carriers of this mutation.	bind
37512	3	8673	5	13	NULL	NULL	NULL	statement 2	Process		results in					LDL cholesterol	Chemical	elevated levels of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_5_826_s_24	9157944	8  Defective apoB-100 has been shown to reduce significantly the binding of apoB-100 to the LDLR, 2 9 10  which results in elevated LDL cholesterol levels in carriers of this mutation.	bind
36643	1	8673	7	NULL	NULL	0	NULL	apoB-100	NULL		bind	NULL				LDLR	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_5_826_s_24	9157944	8  Defective apoB-100 has been shown to reduce significantly the binding of apoB-100 to the LDLR, 2 9 10  which results in elevated LDL cholesterol levels in carriers of this mutation.	bind
36644	2	8673	7	10	NULL	0	NULL	apoB-100		mutant	reduce		significantly			statement 1					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_5_826_s_24	9157944	8  Defective apoB-100 has been shown to reduce significantly the binding of apoB-100 to the LDLR, 2 9 10  which results in elevated LDL cholesterol levels in carriers of this mutation.	bind
36645	3	8673	7	NULL	NULL	0	NULL	statement 2	NULL		results in	NULL				LDL cholesterol	NULL	elevated levels of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_5_826_s_24	9157944	8  Defective apoB-100 has been shown to reduce significantly the binding of apoB-100 to the LDLR, 2 9 10  which results in elevated LDL cholesterol levels in carriers of this mutation.	bind
37513	1	8674	5	13	NULL	NULL	NULL	VLDL	GP		bind					macrophages	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_392_s_205	7538426	8  LPL increases the binding of VLDL and LDL to macrophages, thus enhancing their uptake of triglyceride-rich lipoproteins.	bind
37514	2	8674	5	13	NULL	NULL	NULL	LDL	GP		bind					macrophages	Cell				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_392_s_205	7538426	8  LPL increases the binding of VLDL and LDL to macrophages, thus enhancing their uptake of triglyceride-rich lipoproteins.	bind
37515	3	8674	5	13	NULL	NULL	NULL	LPL	GP		increase					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_392_s_205	7538426	8  LPL increases the binding of VLDL and LDL to macrophages, thus enhancing their uptake of triglyceride-rich lipoproteins.	bind
37516	5	8674	5	13	NULL	NULL	NULL	VLDL	GP		uptake					lipoproteins	GP	triglyceride-rich			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_392_s_205	7538426	8  LPL increases the binding of VLDL and LDL to macrophages, thus enhancing their uptake of triglyceride-rich lipoproteins.	bind
37517	6	8674	5	13	NULL	NULL	NULL	LDL	GP		uptake					lipoproteins	GP	triglyceride-rich			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_392_s_205	7538426	8  LPL increases the binding of VLDL and LDL to macrophages, thus enhancing their uptake of triglyceride-rich lipoproteins.	bind
37518	4	8674	5	13	NULL	NULL	NULL	LPL	GP		increase					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_392_s_205	7538426	8  LPL increases the binding of VLDL and LDL to macrophages, thus enhancing their uptake of triglyceride-rich lipoproteins.	bind
37519	7	8674	5	13	NULL	NULL	NULL	LPL	GP		enhance					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_392_s_205	7538426	8  LPL increases the binding of VLDL and LDL to macrophages, thus enhancing their uptake of triglyceride-rich lipoproteins.	bind
37520	8	8674	5	13	NULL	NULL	NULL	LPL	GP		enhance					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_392_s_205	7538426	8  LPL increases the binding of VLDL and LDL to macrophages, thus enhancing their uptake of triglyceride-rich lipoproteins.	bind
36646	1	8674	7	NULL	NULL	0	NULL	VLDL	NULL		bind	NULL				macrophages	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_392_s_205	7538426	8  LPL increases the binding of VLDL and LDL to macrophages, thus enhancing their uptake of triglyceride-rich lipoproteins.	bind
36647	2	8674	7	NULL	NULL	0	NULL	LDL	NULL		bind	NULL				macrophages	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_392_s_205	7538426	8  LPL increases the binding of VLDL and LDL to macrophages, thus enhancing their uptake of triglyceride-rich lipoproteins.	bind
36648	3	8674	7	NULL	NULL	0	NULL	LPL	NULL		increase	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_392_s_205	7538426	8  LPL increases the binding of VLDL and LDL to macrophages, thus enhancing their uptake of triglyceride-rich lipoproteins.	bind
36649	4	8674	7	NULL	NULL	0	NULL	LPL	NULL		increase	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_392_s_205	7538426	8  LPL increases the binding of VLDL and LDL to macrophages, thus enhancing their uptake of triglyceride-rich lipoproteins.	bind
36650	5	8674	7	10	NULL	0	NULL	VLDL	NULL		uptake of	NULL				lipoproteins	NULL	triglyceride-rich			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_392_s_205	7538426	8  LPL increases the binding of VLDL and LDL to macrophages, thus enhancing their uptake of triglyceride-rich lipoproteins.	bind
36651	6	8674	7	10	NULL	0	NULL	LDL	NULL		uptake of	NULL				lipoproteins	NULL	triglyceride-rich 			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_392_s_205	7538426	8  LPL increases the binding of VLDL and LDL to macrophages, thus enhancing their uptake of triglyceride-rich lipoproteins.	bind
36652	7	8674	7	NULL	NULL	0	NULL	LPL	NULL		enhance	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_392_s_205	7538426	8  LPL increases the binding of VLDL and LDL to macrophages, thus enhancing their uptake of triglyceride-rich lipoproteins.	bind
36653	8	8674	7	NULL	NULL	0	NULL	LPL	NULL		enhance	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_3_392_s_205	7538426	8  LPL increases the binding of VLDL and LDL to macrophages, thus enhancing their uptake of triglyceride-rich lipoproteins.	bind
37521	1	8675	5	13	NULL	NULL	NULL	LDL	GP		activates					p44mapk isoform	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2412_s_22	10521371	8  Recently we demonstrated that LDL activates the 44 kDa and the 42 kDa mitogen-activated protein (MAP) kinase (p44mapk/p42mapk) isoforms as well as elevates [Ca2+]i via a pertussis-toxin (PTX)-sensitive guanosine triphosphate binding protein (Gi protein)-coupled receptor that is independent from its classical receptor.	bind
37522	2	8675	5	13	NULL	NULL	NULL	LDL	GP		activates					p42mapk isoform	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2412_s_22	10521371	8  Recently we demonstrated that LDL activates the 44 kDa and the 42 kDa mitogen-activated protein (MAP) kinase (p44mapk/p42mapk) isoforms as well as elevates [Ca2+]i via a pertussis-toxin (PTX)-sensitive guanosine triphosphate binding protein (Gi protein)-coupled receptor that is independent from its classical receptor.	bind
37523	3	8675	5	13	NULL	NULL	NULL	p44mapk	GP		is					44 kDa mitogen-activated protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2412_s_22	10521371	8  Recently we demonstrated that LDL activates the 44 kDa and the 42 kDa mitogen-activated protein (MAP) kinase (p44mapk/p42mapk) isoforms as well as elevates [Ca2+]i via a pertussis-toxin (PTX)-sensitive guanosine triphosphate binding protein (Gi protein)-coupled receptor that is independent from its classical receptor.	bind
37524	4	8675	5	13	NULL	NULL	NULL	p42mapk	GP		is					42 kDa mitogen-activated protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2412_s_22	10521371	8  Recently we demonstrated that LDL activates the 44 kDa and the 42 kDa mitogen-activated protein (MAP) kinase (p44mapk/p42mapk) isoforms as well as elevates [Ca2+]i via a pertussis-toxin (PTX)-sensitive guanosine triphosphate binding protein (Gi protein)-coupled receptor that is independent from its classical receptor.	bind
37525	5	8675	5	13	NULL	NULL	NULL	LDL	GP		elevate					[Ca2+]i	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2412_s_22	10521371	8  Recently we demonstrated that LDL activates the 44 kDa and the 42 kDa mitogen-activated protein (MAP) kinase (p44mapk/p42mapk) isoforms as well as elevates [Ca2+]i via a pertussis-toxin (PTX)-sensitive guanosine triphosphate binding protein (Gi protein)-coupled receptor that is independent from its classical receptor.	bind
37526	6	8675	5	13	NULL	NULL	NULL	statement 5	Process		via					Gi protein-coupled receptor	GP	PTX-sensitive			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2412_s_22	10521371	8  Recently we demonstrated that LDL activates the 44 kDa and the 42 kDa mitogen-activated protein (MAP) kinase (p44mapk/p42mapk) isoforms as well as elevates [Ca2+]i via a pertussis-toxin (PTX)-sensitive guanosine triphosphate binding protein (Gi protein)-coupled receptor that is independent from its classical receptor.	bind
37527	7	8675	5	13	NULL	NULL	NULL	Gi protein-coupled receptor	GP	PTX-sensitive	is independent from					classical receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2412_s_22	10521371	8  Recently we demonstrated that LDL activates the 44 kDa and the 42 kDa mitogen-activated protein (MAP) kinase (p44mapk/p42mapk) isoforms as well as elevates [Ca2+]i via a pertussis-toxin (PTX)-sensitive guanosine triphosphate binding protein (Gi protein)-coupled receptor that is independent from its classical receptor.	bind
37528	8	8675	5	13	NULL	NULL	NULL	PTX	Chemical		is					pertussis-toxin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2412_s_22	10521371	8  Recently we demonstrated that LDL activates the 44 kDa and the 42 kDa mitogen-activated protein (MAP) kinase (p44mapk/p42mapk) isoforms as well as elevates [Ca2+]i via a pertussis-toxin (PTX)-sensitive guanosine triphosphate binding protein (Gi protein)-coupled receptor that is independent from its classical receptor.	bind
37529	9	8675	5	13	NULL	NULL	NULL	Gi protein	GP		is					guanosine triphosphate binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2412_s_22	10521371	8  Recently we demonstrated that LDL activates the 44 kDa and the 42 kDa mitogen-activated protein (MAP) kinase (p44mapk/p42mapk) isoforms as well as elevates [Ca2+]i via a pertussis-toxin (PTX)-sensitive guanosine triphosphate binding protein (Gi protein)-coupled receptor that is independent from its classical receptor.	bind
36654	1	8675	7	10	NULL	0	NULL	 LDL			activates					p44mapk isoform					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2412_s_22	10521371	8  Recently we demonstrated that LDL activates the 44 kDa and the 42 kDa mitogen-activated protein (MAP) kinase (p44mapk/p42mapk) isoforms as well as elevates [Ca2+]i via a pertussis-toxin (PTX)-sensitive guanosine triphosphate binding protein (Gi protein)-coupled receptor that is independent from its classical receptor.	bind
36655	2	8675	7	10	NULL	0	NULL	p44mapk isoform			is a type of					MAP kinase					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2412_s_22	10521371	8  Recently we demonstrated that LDL activates the 44 kDa and the 42 kDa mitogen-activated protein (MAP) kinase (p44mapk/p42mapk) isoforms as well as elevates [Ca2+]i via a pertussis-toxin (PTX)-sensitive guanosine triphosphate binding protein (Gi protein)-coupled receptor that is independent from its classical receptor.	bind
36656	3	8675	7	NULL	NULL	0	NULL	LDL	NULL		elevates	NULL				[Ca2+]i 	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2412_s_22	10521371	8  Recently we demonstrated that LDL activates the 44 kDa and the 42 kDa mitogen-activated protein (MAP) kinase (p44mapk/p42mapk) isoforms as well as elevates [Ca2+]i via a pertussis-toxin (PTX)-sensitive guanosine triphosphate binding protein (Gi protein)-coupled receptor that is independent from its classical receptor.	bind
36657	4	8675	7	10	NULL	0	NULL	statement 3	NULL		occurs via	NULL				Gi protein coupled receptor	NULL	PTX-sensitive			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2412_s_22	10521371	8  Recently we demonstrated that LDL activates the 44 kDa and the 42 kDa mitogen-activated protein (MAP) kinase (p44mapk/p42mapk) isoforms as well as elevates [Ca2+]i via a pertussis-toxin (PTX)-sensitive guanosine triphosphate binding protein (Gi protein)-coupled receptor that is independent from its classical receptor.	bind
36658	5	8675	7	NULL	NULL	0	NULL	MAP	NULL		is 	NULL				mitogen-activated protein	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2412_s_22	10521371	8  Recently we demonstrated that LDL activates the 44 kDa and the 42 kDa mitogen-activated protein (MAP) kinase (p44mapk/p42mapk) isoforms as well as elevates [Ca2+]i via a pertussis-toxin (PTX)-sensitive guanosine triphosphate binding protein (Gi protein)-coupled receptor that is independent from its classical receptor.	bind
36659	6	8675	7	NULL	NULL	0	NULL	PTX	NULL		is	NULL				pertussis-toxin 	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2412_s_22	10521371	8  Recently we demonstrated that LDL activates the 44 kDa and the 42 kDa mitogen-activated protein (MAP) kinase (p44mapk/p42mapk) isoforms as well as elevates [Ca2+]i via a pertussis-toxin (PTX)-sensitive guanosine triphosphate binding protein (Gi protein)-coupled receptor that is independent from its classical receptor.	bind
36660	7	8675	7	NULL	NULL	0	NULL	Gi protein	NULL		is	NULL				guanosine triphosphate binding protein 	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2412_s_22	10521371	8  Recently we demonstrated that LDL activates the 44 kDa and the 42 kDa mitogen-activated protein (MAP) kinase (p44mapk/p42mapk) isoforms as well as elevates [Ca2+]i via a pertussis-toxin (PTX)-sensitive guanosine triphosphate binding protein (Gi protein)-coupled receptor that is independent from its classical receptor.	bind
56305	8	8675	7	10	NULL	0	NULL	LDL			activates					p42mapk					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2412_s_22	10521371	8  Recently we demonstrated that LDL activates the 44 kDa and the 42 kDa mitogen-activated protein (MAP) kinase (p44mapk/p42mapk) isoforms as well as elevates [Ca2+]i via a pertussis-toxin (PTX)-sensitive guanosine triphosphate binding protein (Gi protein)-coupled receptor that is independent from its classical receptor.	bind
56306	9	8675	7	10	NULL	0	NULL	p42mapk isoform			is a type of					MAP kinase					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2412_s_22	10521371	8  Recently we demonstrated that LDL activates the 44 kDa and the 42 kDa mitogen-activated protein (MAP) kinase (p44mapk/p42mapk) isoforms as well as elevates [Ca2+]i via a pertussis-toxin (PTX)-sensitive guanosine triphosphate binding protein (Gi protein)-coupled receptor that is independent from its classical receptor.	bind
37531	1	8676	5	13	NULL	NULL	NULL	polycystin-1	GP		bind		may	cytoplasmic tail		heterotrimeric G proteins	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_973_s_19	11891195	8  The cytoplasmic tail of polycystin-1 may bind heterotrimeric G proteins  in vitro, 9  activate the transcription factor AP-1, 10  and have a role in modulating Wnt signaling.	bind
37532	2	8676	5	13	NULL	NULL	NULL	polycystin-1	GP		activates		may	cytoplasmic tail		AP-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_973_s_19	11891195	8  The cytoplasmic tail of polycystin-1 may bind heterotrimeric G proteins  in vitro, 9  activate the transcription factor AP-1, 10  and have a role in modulating Wnt signaling.	bind
37533	3	8676	5	13	NULL	NULL	NULL	AP-1	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_973_s_19	11891195	8  The cytoplasmic tail of polycystin-1 may bind heterotrimeric G proteins  in vitro, 9  activate the transcription factor AP-1, 10  and have a role in modulating Wnt signaling.	bind
37534	4	8676	5	13	NULL	NULL	NULL	polycystin-1	GP		modulates		may	cytoplasmic tail		Wnt signaling	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_973_s_19	11891195	8  The cytoplasmic tail of polycystin-1 may bind heterotrimeric G proteins  in vitro, 9  activate the transcription factor AP-1, 10  and have a role in modulating Wnt signaling.	bind
36661	1	8676	7	NULL	NULL	0	NULL	polycystin-1	NULL		bind	NULL	may	cytoplasmic tail of 		 heterotrimeric G proteins	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_amjpathol_160_3_973_s_19	11891195	8  The cytoplasmic tail of polycystin-1 may bind heterotrimeric G proteins  in vitro, 9  activate the transcription factor AP-1, 10  and have a role in modulating Wnt signaling.	bind
36662	2	8676	7	NULL	NULL	0	NULL	statement 1	NULL		activate	NULL				AP-1	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_3_973_s_19	11891195	8  The cytoplasmic tail of polycystin-1 may bind heterotrimeric G proteins  in vitro, 9  activate the transcription factor AP-1, 10  and have a role in modulating Wnt signaling.	bind
36663	3	8676	7	NULL	NULL	0	NULL	AP-1	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_3_973_s_19	11891195	8  The cytoplasmic tail of polycystin-1 may bind heterotrimeric G proteins  in vitro, 9  activate the transcription factor AP-1, 10  and have a role in modulating Wnt signaling.	bind
36664	4	8676	7	NULL	NULL	0	NULL	statement 2	NULL		modulates	NULL				Wnt signaling	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_3_973_s_19	11891195	8  The cytoplasmic tail of polycystin-1 may bind heterotrimeric G proteins  in vitro, 9  activate the transcription factor AP-1, 10  and have a role in modulating Wnt signaling.	bind
37536	1	8678	5	13	NULL	NULL	NULL	UPA	GP		bind					pro-UPA	GP	inactive			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_693_s_29	9598826	8  UPA can bind to the UPAR in either its inactive proenzyme form (pro-UPA) or active two-chain form without affecting its proteolytic activity.	bind
37537	2	8678	5	13	NULL	NULL	NULL	pro-UPA	GP		is					proenzyme form of UPAR	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_693_s_29	9598826	8  UPA can bind to the UPAR in either its inactive proenzyme form (pro-UPA) or active two-chain form without affecting its proteolytic activity.	bind
37538	3	8678	5	13	NULL	NULL	NULL	UPA	GP		bind					UPAR	GP	active two-chain form of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_693_s_29	9598826	8  UPA can bind to the UPAR in either its inactive proenzyme form (pro-UPA) or active two-chain form without affecting its proteolytic activity.	bind
37539	4	8678	5	13	NULL	NULL	NULL	statement 1	Process		does not effect					UPAR	GP	proteolytic activity of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_693_s_29	9598826	8  UPA can bind to the UPAR in either its inactive proenzyme form (pro-UPA) or active two-chain form without affecting its proteolytic activity.	bind
37540	5	8678	5	13	NULL	NULL	NULL	statement 3	Process		does not effect					UPAR	GP	proteolytic activity of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_693_s_29	9598826	8  UPA can bind to the UPAR in either its inactive proenzyme form (pro-UPA) or active two-chain form without affecting its proteolytic activity.	bind
36665	1	8678	7	NULL	NULL	0	NULL	UPA 	NULL		bind	NULL				UPAR	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_693_s_29	9598826	8  UPA can bind to the UPAR in either its inactive proenzyme form (pro-UPA) or active two-chain form without affecting its proteolytic activity.	bind
36666	2	8678	7	NULL	NULL	0	NULL	pro-UPA	NULL		bind	NULL				UPAR	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_693_s_29	9598826	8  UPA can bind to the UPAR in either its inactive proenzyme form (pro-UPA) or active two-chain form without affecting its proteolytic activity.	bind
36667	3	8678	7	NULL	NULL	0	NULL	pro-UPA	NULL		is	NULL				inactive proenzyme form	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_693_s_29	9598826	8  UPA can bind to the UPAR in either its inactive proenzyme form (pro-UPA) or active two-chain form without affecting its proteolytic activity.	bind
36669	4	8678	7	10	NULL	0	NULL	statement 1			does not affect					UPAR		proteolytic activity of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_693_s_29	9598826	8  UPA can bind to the UPAR in either its inactive proenzyme form (pro-UPA) or active two-chain form without affecting its proteolytic activity.	bind
36670	5	8678	7	10	NULL	0	NULL	statement 2			does not affect					UPAR		proteolytic activity of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_693_s_29	9598826	8  UPA can bind to the UPAR in either its inactive proenzyme form (pro-UPA) or active two-chain form without affecting its proteolytic activity.	bind
37541	1	8679	5	13	NULL	NULL	NULL	sera	OrganismPart		bind		progressively			CL	Chemical	oxidized			NULL	APS patients	NULL	NULL	NULL	NULL	gw60_circulation_103_7_941_s_21	11181467	8  We also showed that a few selected reference sera and affinity-purified aCL-IgG from APS patients progressively bound to CL as it was oxidized but not to a "`reduced"' CL (CLred) analogue that was unable to undergo lipid peroxidation (all 4 unsaturated fatty acids in CLred are hydrogenated to saturated fatty acids).	bind
37542	2	8679	5	13	NULL	NULL	NULL	aCL-IgG	GP		bind		progressively			CL	Chemical	oxidized			NULL	APS patients	NULL	NULL	NULL	NULL	gw60_circulation_103_7_941_s_21	11181467	8  We also showed that a few selected reference sera and affinity-purified aCL-IgG from APS patients progressively bound to CL as it was oxidized but not to a "`reduced"' CL (CLred) analogue that was unable to undergo lipid peroxidation (all 4 unsaturated fatty acids in CLred are hydrogenated to saturated fatty acids).	bind
37543	3	8679	5	13	NULL	NULL	NULL	sera	OrganismPart		does not bind		progressively			CLred	Chemical				NULL	APS patients	NULL	NULL	NULL	NULL	gw60_circulation_103_7_941_s_21	11181467	8  We also showed that a few selected reference sera and affinity-purified aCL-IgG from APS patients progressively bound to CL as it was oxidized but not to a "`reduced"' CL (CLred) analogue that was unable to undergo lipid peroxidation (all 4 unsaturated fatty acids in CLred are hydrogenated to saturated fatty acids).	bind
37544	4	8679	5	13	NULL	NULL	NULL	aCL-IgG	GP		does not bind					CLred	Chemical				NULL	APS patients	NULL	NULL	NULL	NULL	gw60_circulation_103_7_941_s_21	11181467	8  We also showed that a few selected reference sera and affinity-purified aCL-IgG from APS patients progressively bound to CL as it was oxidized but not to a "`reduced"' CL (CLred) analogue that was unable to undergo lipid peroxidation (all 4 unsaturated fatty acids in CLred are hydrogenated to saturated fatty acids).	bind
37545	5	8679	5	13	NULL	NULL	NULL	CLred	Chemical		is					reduced CL	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_7_941_s_21	11181467	8  We also showed that a few selected reference sera and affinity-purified aCL-IgG from APS patients progressively bound to CL as it was oxidized but not to a "`reduced"' CL (CLred) analogue that was unable to undergo lipid peroxidation (all 4 unsaturated fatty acids in CLred are hydrogenated to saturated fatty acids).	bind
37546	6	8679	5	13	NULL	NULL	NULL	CLred	Chemical		does not undergo					lipid peroxidation	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_7_941_s_21	11181467	8  We also showed that a few selected reference sera and affinity-purified aCL-IgG from APS patients progressively bound to CL as it was oxidized but not to a "`reduced"' CL (CLred) analogue that was unable to undergo lipid peroxidation (all 4 unsaturated fatty acids in CLred are hydrogenated to saturated fatty acids).	bind
37547	7	8679	5	13	NULL	NULL	NULL	CLred	Chemical	unsaturated fatty acids in	is hydrogenated to					CLred	Chemical	saturated fatty acids in			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_7_941_s_21	11181467	8  We also showed that a few selected reference sera and affinity-purified aCL-IgG from APS patients progressively bound to CL as it was oxidized but not to a "`reduced"' CL (CLred) analogue that was unable to undergo lipid peroxidation (all 4 unsaturated fatty acids in CLred are hydrogenated to saturated fatty acids).	bind
36671	1	8679	7	10	NULL	0	NULL	 aCL-IgG			binds		progressively			CL		oxidized 			NULL	APS patients	NULL	NULL	NULL	NULL	gw60_circulation_103_7_941_s_21	11181467	8  We also showed that a few selected reference sera and affinity-purified aCL-IgG from APS patients progressively bound to CL as it was oxidized but not to a "`reduced"' CL (CLred) analogue that was unable to undergo lipid peroxidation (all 4 unsaturated fatty acids in CLred are hydrogenated to saturated fatty acids).	bind
36672	2	8679	7	NULL	NULL	0	NULL	aCL-IgG	NULL		does not bind	NULL				CLred analogue	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_7_941_s_21	11181467	8  We also showed that a few selected reference sera and affinity-purified aCL-IgG from APS patients progressively bound to CL as it was oxidized but not to a "`reduced"' CL (CLred) analogue that was unable to undergo lipid peroxidation (all 4 unsaturated fatty acids in CLred are hydrogenated to saturated fatty acids).	bind
36673	3	8679	7	NULL	NULL	0	NULL	CLred	NULL		is	NULL				reduced CL	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_7_941_s_21	11181467	8  We also showed that a few selected reference sera and affinity-purified aCL-IgG from APS patients progressively bound to CL as it was oxidized but not to a "`reduced"' CL (CLred) analogue that was unable to undergo lipid peroxidation (all 4 unsaturated fatty acids in CLred are hydrogenated to saturated fatty acids).	bind
36674	4	8679	7	10	NULL	0	NULL	CLred			does not undergo					lipid peroxidation					NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_7_941_s_21	11181467	8  We also showed that a few selected reference sera and affinity-purified aCL-IgG from APS patients progressively bound to CL as it was oxidized but not to a "`reduced"' CL (CLred) analogue that was unable to undergo lipid peroxidation (all 4 unsaturated fatty acids in CLred are hydrogenated to saturated fatty acids).	bind
36675	5	8679	7	10	NULL	0	NULL	CLred	NULL	unsaturated fatty acids in	hydrogenated to	NULL				saturated fatty acids	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_7_941_s_21	11181467	8  We also showed that a few selected reference sera and affinity-purified aCL-IgG from APS patients progressively bound to CL as it was oxidized but not to a "`reduced"' CL (CLred) analogue that was unable to undergo lipid peroxidation (all 4 unsaturated fatty acids in CLred are hydrogenated to saturated fatty acids).	bind
56307	6	8679	7	10	NULL	0	NULL	sera			bind		progressively			CL		oxidized			NULL	APS patients	0	NULL	NULL	NULL	gw60_circulation_103_7_941_s_21	11181467	8  We also showed that a few selected reference sera and affinity-purified aCL-IgG from APS patients progressively bound to CL as it was oxidized but not to a "`reduced"' CL (CLred) analogue that was unable to undergo lipid peroxidation (all 4 unsaturated fatty acids in CLred are hydrogenated to saturated fatty acids).	bind
56310	7	8679	7	10	NULL	0	NULL	sera			does not bind		progressively			CLred					NULL	APS patients	0	NULL	NULL	NULL	gw60_circulation_103_7_941_s_21	11181467	8  We also showed that a few selected reference sera and affinity-purified aCL-IgG from APS patients progressively bound to CL as it was oxidized but not to a "`reduced"' CL (CLred) analogue that was unable to undergo lipid peroxidation (all 4 unsaturated fatty acids in CLred are hydrogenated to saturated fatty acids).	bind
37722	1	8680	5	13	NULL	NULL	NULL	alphavbeta8	GP		bind					latent TGF-beta	GP		RGD sequence of LAP		NULL	lung cancer cell lines	NULL	NULL	NULL	NULL	gw60_amjpathol_163_2_533_s_19	12875973	8  We have recently shown in lung cancer cell lines that alphavbeta8 binds to the RGD sequence of the LAP of latent TGF-beta and mediates activation of the latent TGF-beta complex through a mechanism that is dependent on the transmembrane protease, MT1-MMP.	bind
37723	2	8680	5	13	NULL	NULL	NULL	statement 1	GP		mediate					latent TGF-beta complex 	GP	activation of			NULL	lung cancer cell lines	NULL	NULL	NULL	NULL	gw60_amjpathol_163_2_533_s_19	12875973	8  We have recently shown in lung cancer cell lines that alphavbeta8 binds to the RGD sequence of the LAP of latent TGF-beta and mediates activation of the latent TGF-beta complex through a mechanism that is dependent on the transmembrane protease, MT1-MMP.	bind
37724	3	8680	5	13	NULL	NULL	NULL	statement 2	Process		is dependent on					MT1-MMP	GP				NULL	lung cancer cell lines	NULL	NULL	NULL	NULL	gw60_amjpathol_163_2_533_s_19	12875973	8  We have recently shown in lung cancer cell lines that alphavbeta8 binds to the RGD sequence of the LAP of latent TGF-beta and mediates activation of the latent TGF-beta complex through a mechanism that is dependent on the transmembrane protease, MT1-MMP.	bind
37725	4	8680	5	13	NULL	NULL	NULL	MT1-MMP	GP		is a type of					transmembrane protease	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_163_2_533_s_19	12875973	8  We have recently shown in lung cancer cell lines that alphavbeta8 binds to the RGD sequence of the LAP of latent TGF-beta and mediates activation of the latent TGF-beta complex through a mechanism that is dependent on the transmembrane protease, MT1-MMP.	bind
36676	1	8680	7	NULL	NULL	0	NULL	alphavbeta8	NULL		binds to	NULL				latent TGF-beta	NULL		RGD sequence of the LAP		NULL	lung cancer cell lines	0	NULL	NULL	NULL	gw60_amjpathol_163_2_533_s_19	12875973	8  We have recently shown in lung cancer cell lines that alphavbeta8 binds to the RGD sequence of the LAP of latent TGF-beta and mediates activation of the latent TGF-beta complex through a mechanism that is dependent on the transmembrane protease, MT1-MMP.	bind
36677	2	8680	7	NULL	NULL	0	NULL	statement 1	NULL		mediates	NULL				latent TGF-beta complex	NULL	activation of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_163_2_533_s_19	12875973	8  We have recently shown in lung cancer cell lines that alphavbeta8 binds to the RGD sequence of the LAP of latent TGF-beta and mediates activation of the latent TGF-beta complex through a mechanism that is dependent on the transmembrane protease, MT1-MMP.	bind
36678	3	8680	7	NULL	NULL	0	NULL	statement 2	NULL		depends on	NULL				MT1-MMP	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_163_2_533_s_19	12875973	8  We have recently shown in lung cancer cell lines that alphavbeta8 binds to the RGD sequence of the LAP of latent TGF-beta and mediates activation of the latent TGF-beta complex through a mechanism that is dependent on the transmembrane protease, MT1-MMP.	bind
36679	4	8680	7	NULL	NULL	0	NULL	MT1-MMP	NULL		is a type of	NULL				transmembrane protease	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_163_2_533_s_19	12875973	8  We have recently shown in lung cancer cell lines that alphavbeta8 binds to the RGD sequence of the LAP of latent TGF-beta and mediates activation of the latent TGF-beta complex through a mechanism that is dependent on the transmembrane protease, MT1-MMP.	bind
37726	1	8682	5	13	NULL	NULL	NULL	NP-1	GP		is					neuropilin-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_3_358_s_25	11457758	8 -  10 Specific isoforms of VEGF and PlGF and both isoforms of VEGF-B bind to neuropilin-1 (NP-1).	bind
37727	2	8682	5	13	NULL	NULL	NULL	VEGF isoform	GP		bind					NP-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_3_358_s_25	11457758	8 -  10 Specific isoforms of VEGF and PlGF and both isoforms of VEGF-B bind to neuropilin-1 (NP-1).	bind
37728	3	8682	5	13	NULL	NULL	NULL	PIGF isoform	GP		bind					NP-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_3_358_s_25	11457758	8 -  10 Specific isoforms of VEGF and PlGF and both isoforms of VEGF-B bind to neuropilin-1 (NP-1).	bind
37729	4	8682	5	13	NULL	NULL	NULL	isoforms of VEGF-B	GP		bind					NP-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_3_358_s_25	11457758	8 -  10 Specific isoforms of VEGF and PlGF and both isoforms of VEGF-B bind to neuropilin-1 (NP-1).	bind
36683	1	8682	7	NULL	NULL	0	NULL	VEGF isoform	NULL		bind	NULL				NP-1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_3_358_s_25	11457758	8 -  10 Specific isoforms of VEGF and PlGF and both isoforms of VEGF-B bind to neuropilin-1 (NP-1).	bind
36684	2	8682	7	NULL	NULL	0	NULL	PIGF isoform	NULL		bind	NULL				NP-1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_104_3_358_s_25	11457758	8 -  10 Specific isoforms of VEGF and PlGF and both isoforms of VEGF-B bind to neuropilin-1 (NP-1).	bind
36685	3	8682	7	NULL	NULL	0	NULL	VEGF-B	NULL		bind	NULL				NP-1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_104_3_358_s_25	11457758	8 -  10 Specific isoforms of VEGF and PlGF and both isoforms of VEGF-B bind to neuropilin-1 (NP-1).	bind
36686	4	8682	7	NULL	NULL	0	NULL	NP-1	NULL		is	NULL				neuropilin-1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_104_3_358_s_25	11457758	8 -  10 Specific isoforms of VEGF and PlGF and both isoforms of VEGF-B bind to neuropilin-1 (NP-1).	bind
37730	1	8683	5	13	NULL	NULL	NULL	paraoxonase	GP		bind					HDL	GP	large			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_10_1243_s_170	8857920	8 14  While the relation between paraoxonase and HDL may reflect enzyme binding to large HDL (with apoA-I), 14  this would not account for the reported associations with plasma TG or apoB levels that others have reported.	bind
46798	2	8683	5	13	NULL	NULL	NULL	HDL	GP	large	contains					apoA-I	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_10_1243_s_170	8857920	8 14  While the relation between paraoxonase and HDL may reflect enzyme binding to large HDL (with apoA-I), 14  this would not account for the reported associations with plasma TG or apoB levels that others have reported.	bind
36687	1	8683	7	10	NULL	0	NULL	paraoxonase			bind					HDL		large			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_10_1243_s_170	8857920	8 14  While the relation between paraoxonase and HDL may reflect enzyme binding to large HDL (with apoA-I), 14  this would not account for the reported associations with plasma TG or apoB levels that others have reported.	bind
36688	2	8683	7	10	NULL	0	NULL	HDL		large	contains					apoA-I					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_10_1243_s_170	8857920	8 14  While the relation between paraoxonase and HDL may reflect enzyme binding to large HDL (with apoA-I), 14  this would not account for the reported associations with plasma TG or apoB levels that others have reported.	bind
37731	1	8685	5	13	NULL	NULL	NULL	UPA	GP		bind					UPAR	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_693_s_51	9598826	8 38  The binding of UPA to its receptor is rather species specific, since human UPA cannot bind to mouse UPAR and vice versa.	bind
37732	2	8685	5	13	NULL	NULL	NULL	UPA	GP	human	does not bind					UPAR	GP	mouse			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_693_s_51	9598826	8 38  The binding of UPA to its receptor is rather species specific, since human UPA cannot bind to mouse UPAR and vice versa.	bind
37733	3	8685	5	13	NULL	NULL	NULL	UPA	GP	mouse	does not bind					UPAR	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_693_s_51	9598826	8 38  The binding of UPA to its receptor is rather species specific, since human UPA cannot bind to mouse UPAR and vice versa.	bind
36877	1	8685	7	NULL	NULL	0	NULL	UPA	NULL		bind	NULL				UPA receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_693_s_51	9598826	8 38  The binding of UPA to its receptor is rather species specific, since human UPA cannot bind to mouse UPAR and vice versa.	bind
36879	2	8685	7	10	NULL	0	NULL	UPA		human	does not bind					UPAR		mouse			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_693_s_51	9598826	8 38  The binding of UPA to its receptor is rather species specific, since human UPA cannot bind to mouse UPAR and vice versa.	bind
36880	3	8685	7	10	NULL	0	NULL	UPA		mouse	does not bind					UPAR		human			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_5_693_s_51	9598826	8 38  The binding of UPA to its receptor is rather species specific, since human UPA cannot bind to mouse UPAR and vice versa.	bind
37734	1	8686	5	13	NULL	NULL	NULL	IGF-1	GP		bind					smooth muscle cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_6_1689_s_29	7882475	8 9  In addition, [[ fibroblast growth factor ]] increases the binding of IGF-1 to smooth muscle cells, promoting the growth stimulation of IGF-1.	bind
37735	2	8686	5	13	NULL	NULL	NULL	fibroblast growth factor	GP		increase					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_6_1689_s_29	7882475	8 9  In addition, [[ fibroblast growth factor ]] increases the binding of IGF-1 to smooth muscle cells, promoting the growth stimulation of IGF-1.	bind
37736	3	8686	5	13	NULL	NULL	NULL	statement 2	Process		promotes					IGF-1	GP	growth stimulation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_91_6_1689_s_29	7882475	8 9  In addition, [[ fibroblast growth factor ]] increases the binding of IGF-1 to smooth muscle cells, promoting the growth stimulation of IGF-1.	bind
36881	1	8686	7	NULL	NULL	0	NULL	IGF-1	NULL		bind	NULL				smooth muscle cells	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_91_6_1689_s_29	7882475	8 9  In addition, [[ fibroblast growth factor ]] increases the binding of IGF-1 to smooth muscle cells, promoting the growth stimulation of IGF-1.	bind
36882	2	8686	7	NULL	NULL	0	NULL	 fibroblast growth factor	NULL		increase	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_91_6_1689_s_29	7882475	8 9  In addition, [[ fibroblast growth factor ]] increases the binding of IGF-1 to smooth muscle cells, promoting the growth stimulation of IGF-1.	bind
36883	3	8686	7	NULL	NULL	0	NULL	fibroblast growth factor	NULL		promote	NULL				IGF-1	NULL	growth stimulation of			NULL		0	NULL	NULL	NULL	gw60_circulation_91_6_1689_s_29	7882475	8 9  In addition, [[ fibroblast growth factor ]] increases the binding of IGF-1 to smooth muscle cells, promoting the growth stimulation of IGF-1.	bind
37737	1	8687	5	13	NULL	NULL	NULL	NIF	GP		bind					CD11b integrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_3_254_s_19	10926878	8 9 10 11  We showed that NIF can bind to both CD11b and CD11a integrins and thereby prevent PMN adhesion to endothelial cells to a degree equivalent to anti-CD18 monoclonal antibodies.	bind
37738	2	8687	5	13	NULL	NULL	NULL	NIF	GP		bind					CD11a integrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_3_254_s_19	10926878	8 9 10 11  We showed that NIF can bind to both CD11b and CD11a integrins and thereby prevent PMN adhesion to endothelial cells to a degree equivalent to anti-CD18 monoclonal antibodies.	bind
37739	3	8687	5	13	NULL	NULL	NULL	PMN	Cell		adhere to					endothelial cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_3_254_s_19	10926878	8 9 10 11  We showed that NIF can bind to both CD11b and CD11a integrins and thereby prevent PMN adhesion to endothelial cells to a degree equivalent to anti-CD18 monoclonal antibodies.	bind
37740	4	8687	5	13	NULL	NULL	NULL	PMN	Cell		adhere to					anti-CD18 monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_3_254_s_19	10926878	8 9 10 11  We showed that NIF can bind to both CD11b and CD11a integrins and thereby prevent PMN adhesion to endothelial cells to a degree equivalent to anti-CD18 monoclonal antibodies.	bind
37741	5	8687	5	13	NULL	NULL	NULL	statement 1	Process		prevents					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_3_254_s_19	10926878	8 9 10 11  We showed that NIF can bind to both CD11b and CD11a integrins and thereby prevent PMN adhesion to endothelial cells to a degree equivalent to anti-CD18 monoclonal antibodies.	bind
37742	6	8687	5	13	NULL	NULL	NULL	statement 2	Process		prevents					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_3_254_s_19	10926878	8 9 10 11  We showed that NIF can bind to both CD11b and CD11a integrins and thereby prevent PMN adhesion to endothelial cells to a degree equivalent to anti-CD18 monoclonal antibodies.	bind
37743	7	8687	5	13	NULL	NULL	NULL	statement 1	Process		prevents					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_3_254_s_19	10926878	8 9 10 11  We showed that NIF can bind to both CD11b and CD11a integrins and thereby prevent PMN adhesion to endothelial cells to a degree equivalent to anti-CD18 monoclonal antibodies.	bind
37744	8	8687	5	13	NULL	NULL	NULL	statement 2	Process		prevents					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_3_254_s_19	10926878	8 9 10 11  We showed that NIF can bind to both CD11b and CD11a integrins and thereby prevent PMN adhesion to endothelial cells to a degree equivalent to anti-CD18 monoclonal antibodies.	bind
36884	1	8687	7	NULL	NULL	0	NULL	 NIF	NULL		bind	NULL				CD11b integrin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_3_254_s_19	10926878	8 9 10 11  We showed that NIF can bind to both CD11b and CD11a integrins and thereby prevent PMN adhesion to endothelial cells to a degree equivalent to anti-CD18 monoclonal antibodies.	bind
36885	2	8687	7	NULL	NULL	0	NULL	NIF	NULL		bind	NULL				CD11a integrin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_3_254_s_19	10926878	8 9 10 11  We showed that NIF can bind to both CD11b and CD11a integrins and thereby prevent PMN adhesion to endothelial cells to a degree equivalent to anti-CD18 monoclonal antibodies.	bind
36886	3	8687	7	NULL	NULL	0	NULL	PMN	NULL		adhere to	NULL				endothelial cells	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_3_254_s_19	10926878	8 9 10 11  We showed that NIF can bind to both CD11b and CD11a integrins and thereby prevent PMN adhesion to endothelial cells to a degree equivalent to anti-CD18 monoclonal antibodies.	bind
36887	4	8687	7	NULL	NULL	0	NULL	PMN	NULL		adhere to	NULL				anti-CD18 monoclonal antibodies	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_3_254_s_19	10926878	8 9 10 11  We showed that NIF can bind to both CD11b and CD11a integrins and thereby prevent PMN adhesion to endothelial cells to a degree equivalent to anti-CD18 monoclonal antibodies.	bind
36888	5	8687	7	NULL	NULL	0	NULL	statement 1	NULL		prevent	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_3_254_s_19	10926878	8 9 10 11  We showed that NIF can bind to both CD11b and CD11a integrins and thereby prevent PMN adhesion to endothelial cells to a degree equivalent to anti-CD18 monoclonal antibodies.	bind
36889	6	8687	7	NULL	NULL	0	NULL	statement 2	NULL		prevent	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_3_254_s_19	10926878	8 9 10 11  We showed that NIF can bind to both CD11b and CD11a integrins and thereby prevent PMN adhesion to endothelial cells to a degree equivalent to anti-CD18 monoclonal antibodies.	bind
36890	7	8687	7	NULL	NULL	0	NULL	statement 1	NULL		prevent	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_3_254_s_19	10926878	8 9 10 11  We showed that NIF can bind to both CD11b and CD11a integrins and thereby prevent PMN adhesion to endothelial cells to a degree equivalent to anti-CD18 monoclonal antibodies.	bind
36891	8	8687	7	NULL	NULL	0	NULL	statement 2	NULL		prevent	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_3_254_s_19	10926878	8 9 10 11  We showed that NIF can bind to both CD11b and CD11a integrins and thereby prevent PMN adhesion to endothelial cells to a degree equivalent to anti-CD18 monoclonal antibodies.	bind
37745	1	8688	5	13	NULL	NULL	NULL	VEGF-E	GP		bind		selectively			VEGFR-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_85_11_992_s_26	10571529	8 9 10 11 18  VEGF-E binds selectively to VEGFR-2.	bind
36892	1	8688	7	NULL	NULL	0	NULL	VEGF-E 	NULL		binds	NULL	selectively			VEGFR-2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_85_11_992_s_26	10571529	8 9 10 11 18  VEGF-E binds selectively to VEGFR-2.	bind
37746	1	8689	5	13	NULL	NULL	NULL	HB-EGF	GP		bind					EGF receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_2_263_s_153	8756003	8 9 12 13 14  For example, treatment of bovine SMCs with either heparitinase (which degrades heparan sulfate chains), chlorate (which inhibits sulfation of glycosaminoglycans), or a synthetic peptide corresponding to the heparin-binding domain of HB-EGF inhibits HB-EGF binding to the EGF receptor as well as HB-EGF - stimulated cell migration.	bind
37747	2	8689	5	13	NULL	NULL	NULL	HB-EGF	GP		stimulate					cell migration	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_2_263_s_153	8756003	8 9 12 13 14  For example, treatment of bovine SMCs with either heparitinase (which degrades heparan sulfate chains), chlorate (which inhibits sulfation of glycosaminoglycans), or a synthetic peptide corresponding to the heparin-binding domain of HB-EGF inhibits HB-EGF binding to the EGF receptor as well as HB-EGF - stimulated cell migration.	bind
37748	3	8689	5	13	NULL	NULL	NULL	heparitinase	GP	treatment	inhibit					statement 1	Process				NULL	bovine SMCs	NULL	NULL	NULL	NULL	gw60_circulationres_79_2_263_s_153	8756003	8 9 12 13 14  For example, treatment of bovine SMCs with either heparitinase (which degrades heparan sulfate chains), chlorate (which inhibits sulfation of glycosaminoglycans), or a synthetic peptide corresponding to the heparin-binding domain of HB-EGF inhibits HB-EGF binding to the EGF receptor as well as HB-EGF - stimulated cell migration.	bind
37749	4	8689	5	13	NULL	NULL	NULL	heparitinase	GP	treatment	inhibit					statement 2	Process				NULL	bovine SMCs	NULL	NULL	NULL	NULL	gw60_circulationres_79_2_263_s_153	8756003	8 9 12 13 14  For example, treatment of bovine SMCs with either heparitinase (which degrades heparan sulfate chains), chlorate (which inhibits sulfation of glycosaminoglycans), or a synthetic peptide corresponding to the heparin-binding domain of HB-EGF inhibits HB-EGF binding to the EGF receptor as well as HB-EGF - stimulated cell migration.	bind
37750	5	8689	5	13	NULL	NULL	NULL	heparitinase	GP		degrade					heparan sulfate chains	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_2_263_s_153	8756003	8 9 12 13 14  For example, treatment of bovine SMCs with either heparitinase (which degrades heparan sulfate chains), chlorate (which inhibits sulfation of glycosaminoglycans), or a synthetic peptide corresponding to the heparin-binding domain of HB-EGF inhibits HB-EGF binding to the EGF receptor as well as HB-EGF - stimulated cell migration.	bind
37751	6	8689	5	13	NULL	NULL	NULL	chlorate	Chemical	treatment	inhibit					statement 1	Process				NULL	bovine SMCs	NULL	NULL	NULL	NULL	gw60_circulationres_79_2_263_s_153	8756003	8 9 12 13 14  For example, treatment of bovine SMCs with either heparitinase (which degrades heparan sulfate chains), chlorate (which inhibits sulfation of glycosaminoglycans), or a synthetic peptide corresponding to the heparin-binding domain of HB-EGF inhibits HB-EGF binding to the EGF receptor as well as HB-EGF - stimulated cell migration.	bind
37752	7	8689	5	13	NULL	NULL	NULL	chlorate	Chemical	treatment	inhibit					statement 2	Process				NULL	bovine SMCs	NULL	NULL	NULL	NULL	gw60_circulationres_79_2_263_s_153	8756003	8 9 12 13 14  For example, treatment of bovine SMCs with either heparitinase (which degrades heparan sulfate chains), chlorate (which inhibits sulfation of glycosaminoglycans), or a synthetic peptide corresponding to the heparin-binding domain of HB-EGF inhibits HB-EGF binding to the EGF receptor as well as HB-EGF - stimulated cell migration.	bind
37753	8	8689	5	13	NULL	NULL	NULL	chlorate	Chemical		inhibit					glycosaminoglycans	GP	sulfation of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_2_263_s_153	8756003	8 9 12 13 14  For example, treatment of bovine SMCs with either heparitinase (which degrades heparan sulfate chains), chlorate (which inhibits sulfation of glycosaminoglycans), or a synthetic peptide corresponding to the heparin-binding domain of HB-EGF inhibits HB-EGF binding to the EGF receptor as well as HB-EGF - stimulated cell migration.	bind
37754	9	8689	5	13	NULL	NULL	NULL	synthetic peptide	GP		corresponds to					HB-EGF	GP		heparin-binding domain		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_79_2_263_s_153	8756003	8 9 12 13 14  For example, treatment of bovine SMCs with either heparitinase (which degrades heparan sulfate chains), chlorate (which inhibits sulfation of glycosaminoglycans), or a synthetic peptide corresponding to the heparin-binding domain of HB-EGF inhibits HB-EGF binding to the EGF receptor as well as HB-EGF - stimulated cell migration.	bind
37755	10	8689	5	13	NULL	NULL	NULL	statement 9	Process	treatment	inhibit					statement 1	Process				NULL	bovine SMCs	NULL	NULL	NULL	NULL	gw60_circulationres_79_2_263_s_153	8756003	8 9 12 13 14  For example, treatment of bovine SMCs with either heparitinase (which degrades heparan sulfate chains), chlorate (which inhibits sulfation of glycosaminoglycans), or a synthetic peptide corresponding to the heparin-binding domain of HB-EGF inhibits HB-EGF binding to the EGF receptor as well as HB-EGF - stimulated cell migration.	bind
37756	11	8689	5	13	NULL	NULL	NULL	statement 9	Process	treatment	inhibit					statement 2	Process				NULL	bovine SMCs	NULL	NULL	NULL	NULL	gw60_circulationres_79_2_263_s_153	8756003	8 9 12 13 14  For example, treatment of bovine SMCs with either heparitinase (which degrades heparan sulfate chains), chlorate (which inhibits sulfation of glycosaminoglycans), or a synthetic peptide corresponding to the heparin-binding domain of HB-EGF inhibits HB-EGF binding to the EGF receptor as well as HB-EGF - stimulated cell migration.	bind
36893	1	8689	7	NULL	NULL	0	NULL	HB-EGF	NULL		bind	NULL				EGF receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_79_2_263_s_153	8756003	8 9 12 13 14  For example, treatment of bovine SMCs with either heparitinase (which degrades heparan sulfate chains), chlorate (which inhibits sulfation of glycosaminoglycans), or a synthetic peptide corresponding to the heparin-binding domain of HB-EGF inhibits HB-EGF binding to the EGF receptor as well as HB-EGF - stimulated cell migration.	bind
36894	2	8689	7	NULL	NULL	0	NULL	HB-EGF	NULL		stimulate	NULL				cell migration	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_79_2_263_s_153	8756003	8 9 12 13 14  For example, treatment of bovine SMCs with either heparitinase (which degrades heparan sulfate chains), chlorate (which inhibits sulfation of glycosaminoglycans), or a synthetic peptide corresponding to the heparin-binding domain of HB-EGF inhibits HB-EGF binding to the EGF receptor as well as HB-EGF - stimulated cell migration.	bind
36895	3	8689	7	NULL	NULL	0	NULL	heparitinase 	NULL		degrades	NULL				heparan sulfate chains	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_79_2_263_s_153	8756003	8 9 12 13 14  For example, treatment of bovine SMCs with either heparitinase (which degrades heparan sulfate chains), chlorate (which inhibits sulfation of glycosaminoglycans), or a synthetic peptide corresponding to the heparin-binding domain of HB-EGF inhibits HB-EGF binding to the EGF receptor as well as HB-EGF - stimulated cell migration.	bind
36896	4	8689	7	NULL	NULL	0	NULL	heparitinase	NULL		inhibits	NULL				statement 1	NULL				NULL	bovine SMCs	0	NULL	NULL	NULL	gw60_circulationres_79_2_263_s_153	8756003	8 9 12 13 14  For example, treatment of bovine SMCs with either heparitinase (which degrades heparan sulfate chains), chlorate (which inhibits sulfation of glycosaminoglycans), or a synthetic peptide corresponding to the heparin-binding domain of HB-EGF inhibits HB-EGF binding to the EGF receptor as well as HB-EGF - stimulated cell migration.	bind
36897	5	8689	7	NULL	NULL	0	NULL	chlorate	NULL		inhibits	NULL				 glycosaminoglycans	NULL	sulfation of			NULL		0	NULL	NULL	NULL	gw60_circulationres_79_2_263_s_153	8756003	8 9 12 13 14  For example, treatment of bovine SMCs with either heparitinase (which degrades heparan sulfate chains), chlorate (which inhibits sulfation of glycosaminoglycans), or a synthetic peptide corresponding to the heparin-binding domain of HB-EGF inhibits HB-EGF binding to the EGF receptor as well as HB-EGF - stimulated cell migration.	bind
36898	6	8689	7	NULL	NULL	0	NULL	cholrate	NULL		inhibits	NULL				statement 1	NULL				NULL	bovine SMCs	0	NULL	NULL	NULL	gw60_circulationres_79_2_263_s_153	8756003	8 9 12 13 14  For example, treatment of bovine SMCs with either heparitinase (which degrades heparan sulfate chains), chlorate (which inhibits sulfation of glycosaminoglycans), or a synthetic peptide corresponding to the heparin-binding domain of HB-EGF inhibits HB-EGF binding to the EGF receptor as well as HB-EGF - stimulated cell migration.	bind
36899	7	8689	7	NULL	NULL	0	NULL	heparitinase	NULL		inhibits	NULL				statement 2	NULL				NULL	bovine SMCs	0	NULL	NULL	NULL	gw60_circulationres_79_2_263_s_153	8756003	8 9 12 13 14  For example, treatment of bovine SMCs with either heparitinase (which degrades heparan sulfate chains), chlorate (which inhibits sulfation of glycosaminoglycans), or a synthetic peptide corresponding to the heparin-binding domain of HB-EGF inhibits HB-EGF binding to the EGF receptor as well as HB-EGF - stimulated cell migration.	bind
36900	8	8689	7	NULL	NULL	0	NULL	chlorate	NULL		inhibits	NULL				statement 2	NULL				NULL	bovine SMCs	0	NULL	NULL	NULL	gw60_circulationres_79_2_263_s_153	8756003	8 9 12 13 14  For example, treatment of bovine SMCs with either heparitinase (which degrades heparan sulfate chains), chlorate (which inhibits sulfation of glycosaminoglycans), or a synthetic peptide corresponding to the heparin-binding domain of HB-EGF inhibits HB-EGF binding to the EGF receptor as well as HB-EGF - stimulated cell migration.	bind
36901	9	8689	7	NULL	NULL	0	NULL	synthetic peptide 	NULL		corresponds to	NULL				HB-EGF	NULL		heparin-binding domain of		NULL		0	NULL	NULL	NULL	gw60_circulationres_79_2_263_s_153	8756003	8 9 12 13 14  For example, treatment of bovine SMCs with either heparitinase (which degrades heparan sulfate chains), chlorate (which inhibits sulfation of glycosaminoglycans), or a synthetic peptide corresponding to the heparin-binding domain of HB-EGF inhibits HB-EGF binding to the EGF receptor as well as HB-EGF - stimulated cell migration.	bind
36902	10	8689	7	NULL	NULL	0	NULL	Synthetic peptide	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_79_2_263_s_153	8756003	8 9 12 13 14  For example, treatment of bovine SMCs with either heparitinase (which degrades heparan sulfate chains), chlorate (which inhibits sulfation of glycosaminoglycans), or a synthetic peptide corresponding to the heparin-binding domain of HB-EGF inhibits HB-EGF binding to the EGF receptor as well as HB-EGF - stimulated cell migration.	bind
37757	1	8690	5	13	NULL	NULL	NULL	FasL	GP	membrane-bound	bind					Fas-bearing cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_5_1783_s_21	12414525	8 Apoptosis is induced when membrane-bound or soluble FasL binds to Fas-bearing cells.	bind
37758	2	8690	5	13	NULL	NULL	NULL	statement 1	Process		induce					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_5_1783_s_21	12414525	8 Apoptosis is induced when membrane-bound or soluble FasL binds to Fas-bearing cells.	bind
37759	3	8690	5	13	NULL	NULL	NULL	FasL	GP	soluble	bind					Fas-bearing cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_5_1783_s_21	12414525	8 Apoptosis is induced when membrane-bound or soluble FasL binds to Fas-bearing cells.	bind
37760	4	8690	5	13	NULL	NULL	NULL	statement 3	Process		induce					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_5_1783_s_21	12414525	8 Apoptosis is induced when membrane-bound or soluble FasL binds to Fas-bearing cells.	bind
37761	5	8690	5	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_5_1783_s_21	12414525	8 Apoptosis is induced when membrane-bound or soluble FasL binds to Fas-bearing cells.	bind
36903	1	8690	7	NULL	NULL	0	NULL	FasL	NULL	 membrane-bound	binds to	NULL				Fas-bearing cells	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_5_1783_s_21	12414525	8 Apoptosis is induced when membrane-bound or soluble FasL binds to Fas-bearing cells.	bind
36904	2	8690	7	NULL	NULL	0	NULL	FasL	NULL	soluble	binds to	NULL				Fas-bearing cells	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_5_1783_s_21	12414525	8 Apoptosis is induced when membrane-bound or soluble FasL binds to Fas-bearing cells.	bind
36905	3	8690	7	NULL	NULL	0	NULL	statement 1	NULL		induce	NULL				apoptosis	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_5_1783_s_21	12414525	8 Apoptosis is induced when membrane-bound or soluble FasL binds to Fas-bearing cells.	bind
36906	4	8690	7	NULL	NULL	0	NULL	statement 2	NULL		induce	NULL				apoptosis	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_5_1783_s_21	12414525	8 Apoptosis is induced when membrane-bound or soluble FasL binds to Fas-bearing cells.	bind
37762	1	8691	5	13	NULL	NULL	NULL	VWF	GP		bind					GPIb complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_1_14_s_30	11788455	8 Because the binding of VWF to the GPIb complex is known to activate another platelet integrin, alphaIIbbeta3, it is conceivable that it may also activate alpha2beta1.	bind
37763	2	8691	5	13	NULL	NULL	NULL	statement 1	Process		activate					alphaIIbbeta3	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_1_14_s_30	11788455	8 Because the binding of VWF to the GPIb complex is known to activate another platelet integrin, alphaIIbbeta3, it is conceivable that it may also activate alpha2beta1.	bind
37764	3	8691	5	13	NULL	NULL	NULL	alphaIIbbeta3	GP		is a type of					platelet integrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_1_14_s_30	11788455	8 Because the binding of VWF to the GPIb complex is known to activate another platelet integrin, alphaIIbbeta3, it is conceivable that it may also activate alpha2beta1.	bind
37765	4	8691	5	13	NULL	NULL	NULL	statement 1	Process		activate					alpha2beta1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_1_14_s_30	11788455	8 Because the binding of VWF to the GPIb complex is known to activate another platelet integrin, alphaIIbbeta3, it is conceivable that it may also activate alpha2beta1.	bind
36907	1	8691	7	NULL	NULL	0	NULL	VWF	NULL		bind	NULL				GPIb complex 	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_1_14_s_30	11788455	8 Because the binding of VWF to the GPIb complex is known to activate another platelet integrin, alphaIIbbeta3, it is conceivable that it may also activate alpha2beta1.	bind
36908	2	8691	7	NULL	NULL	0	NULL	statement 1	NULL		activate	NULL				alphaIIbbeta3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_1_14_s_30	11788455	8 Because the binding of VWF to the GPIb complex is known to activate another platelet integrin, alphaIIbbeta3, it is conceivable that it may also activate alpha2beta1.	bind
36909	3	8691	7	NULL	NULL	0	NULL	statement 1	NULL		activate	NULL				alpha2beta1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_1_14_s_30	11788455	8 Because the binding of VWF to the GPIb complex is known to activate another platelet integrin, alphaIIbbeta3, it is conceivable that it may also activate alpha2beta1.	bind
36910	4	8691	7	NULL	NULL	0	NULL	alphaIIbbeta3	NULL		is a type of	NULL				platelet integrin	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_1_14_s_30	11788455	8 Because the binding of VWF to the GPIb complex is known to activate another platelet integrin, alphaIIbbeta3, it is conceivable that it may also activate alpha2beta1.	bind
37766	1	8692	5	13	NULL	NULL	NULL	thrombin	GP		bind					thrombomodulin	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_11_2273_s_66	16123318	8 Binding of thrombin to thrombomodulin changes its substrate specificity from fibrinogen to protein C, whereas binding of protein C to EPCR facilitates its cleavage by the thrombomodulin-thrombin complex.	bind
37767	2	8692	5	13	NULL	NULL	NULL	fibrinogen	GP		is substrate for					thrombomodulin	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_11_2273_s_66	16123318	8 Binding of thrombin to thrombomodulin changes its substrate specificity from fibrinogen to protein C, whereas binding of protein C to EPCR facilitates its cleavage by the thrombomodulin-thrombin complex.	bind
37768	3	8692	5	13	NULL	NULL	NULL	protein C	GP		is substrate for					thrombomodulin	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_11_2273_s_66	16123318	8 Binding of thrombin to thrombomodulin changes its substrate specificity from fibrinogen to protein C, whereas binding of protein C to EPCR facilitates its cleavage by the thrombomodulin-thrombin complex.	bind
37769	4	8692	5	13	NULL	NULL	NULL	statement 2	Process		change to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_11_2273_s_66	16123318	8 Binding of thrombin to thrombomodulin changes its substrate specificity from fibrinogen to protein C, whereas binding of protein C to EPCR facilitates its cleavage by the thrombomodulin-thrombin complex.	bind
37770	5	8692	5	13	NULL	NULL	NULL	statement 1	Process		cause					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_11_2273_s_66	16123318	8 Binding of thrombin to thrombomodulin changes its substrate specificity from fibrinogen to protein C, whereas binding of protein C to EPCR facilitates its cleavage by the thrombomodulin-thrombin complex.	bind
37771	6	8692	5	13	NULL	NULL	NULL	protein C	GP		bind					EPCR	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_11_2273_s_66	16123318	8 Binding of thrombin to thrombomodulin changes its substrate specificity from fibrinogen to protein C, whereas binding of protein C to EPCR facilitates its cleavage by the thrombomodulin-thrombin complex.	bind
37772	7	8692	5	13	NULL	NULL	NULL	thrombomodulin-thrombin complex	GP		cleave					protein C	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_11_2273_s_66	16123318	8 Binding of thrombin to thrombomodulin changes its substrate specificity from fibrinogen to protein C, whereas binding of protein C to EPCR facilitates its cleavage by the thrombomodulin-thrombin complex.	bind
37773	8	8692	5	13	NULL	NULL	NULL	statement 6	Process		facilitates					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_11_2273_s_66	16123318	8 Binding of thrombin to thrombomodulin changes its substrate specificity from fibrinogen to protein C, whereas binding of protein C to EPCR facilitates its cleavage by the thrombomodulin-thrombin complex.	bind
36911	1	8692	7	NULL	NULL	0	NULL	thrombin	NULL		bind	NULL				thrombomodulin	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_11_2273_s_66	16123318	8 Binding of thrombin to thrombomodulin changes its substrate specificity from fibrinogen to protein C, whereas binding of protein C to EPCR facilitates its cleavage by the thrombomodulin-thrombin complex.	bind
36912	2	8692	7	NULL	NULL	0	NULL	fibrinogen	NULL		substrate for	NULL				thrombomodulin	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_11_2273_s_66	16123318	8 Binding of thrombin to thrombomodulin changes its substrate specificity from fibrinogen to protein C, whereas binding of protein C to EPCR facilitates its cleavage by the thrombomodulin-thrombin complex.	bind
36913	3	8692	7	NULL	NULL	0	NULL	protein C	NULL		substrate for	NULL				thrombomodulin	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_11_2273_s_66	16123318	8 Binding of thrombin to thrombomodulin changes its substrate specificity from fibrinogen to protein C, whereas binding of protein C to EPCR facilitates its cleavage by the thrombomodulin-thrombin complex.	bind
36914	4	8692	7	NULL	NULL	0	NULL	statement 2	NULL		change to	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_11_2273_s_66	16123318	8 Binding of thrombin to thrombomodulin changes its substrate specificity from fibrinogen to protein C, whereas binding of protein C to EPCR facilitates its cleavage by the thrombomodulin-thrombin complex.	bind
36915	5	8692	7	NULL	NULL	0	NULL	statement 1	NULL		cause	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_11_2273_s_66	16123318	8 Binding of thrombin to thrombomodulin changes its substrate specificity from fibrinogen to protein C, whereas binding of protein C to EPCR facilitates its cleavage by the thrombomodulin-thrombin complex.	bind
36916	6	8692	7	NULL	NULL	0	NULL	protein C	NULL		bind	NULL				EPCR	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_11_2273_s_66	16123318	8 Binding of thrombin to thrombomodulin changes its substrate specificity from fibrinogen to protein C, whereas binding of protein C to EPCR facilitates its cleavage by the thrombomodulin-thrombin complex.	bind
36917	7	8692	7	NULL	NULL	0	NULL	thrombomodulin-thrombin complex	NULL		cleaves	NULL				EPCR	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_11_2273_s_66	16123318	8 Binding of thrombin to thrombomodulin changes its substrate specificity from fibrinogen to protein C, whereas binding of protein C to EPCR facilitates its cleavage by the thrombomodulin-thrombin complex.	bind
36918	8	8692	7	NULL	NULL	0	NULL	statement 6	NULL		facilitates	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_11_2273_s_66	16123318	8 Binding of thrombin to thrombomodulin changes its substrate specificity from fibrinogen to protein C, whereas binding of protein C to EPCR facilitates its cleavage by the thrombomodulin-thrombin complex.	bind
37774	1	8693	5	13	NULL	NULL	NULL	Cbfa1	GP		bind		sequence specifically					proximal		OSE2 element	NULL	Cbfa1-transfected COS1 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_33_25163_s_274	10833509	8 cells and Cbfa1-transfected COS1 cells, showed that Cbfa1 binds to the proximal OSE2 element in a sequence-specific manner.	bind
36919	1	8693	7	NULL	NULL	0	NULL	 Cbfa1	NULL		binds to	NULL	sequence-specific				NULL	proximal		OSE2 element	NULL	Cbfa1-transfected COS1 cells	0	NULL	NULL	NULL	gw60_jbiolchem_275_33_25163_s_274	10833509	8 cells and Cbfa1-transfected COS1 cells, showed that Cbfa1 binds to the proximal OSE2 element in a sequence-specific manner.	bind
37775	1	8694	5	13	NULL	NULL	NULL	BMP-7	GP		bind					HS	Chemical	endogenous			NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_308_4_858_s_170	12927798	8 cells and that exogenous heparin competitively inhibits BMP-7 binding to endogenous HS.	bind
37776	2	8694	5	13	NULL	NULL	NULL	heparin	Chemical	exogenous	inhibit		competitively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_308_4_858_s_170	12927798	8 cells and that exogenous heparin competitively inhibits BMP-7 binding to endogenous HS.	bind
36920	1	8694	7	10	NULL	0	NULL	BMP-7	NULL		bind	NULL				HS	NULL	endogenous 			NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_308_4_858_s_170	12927798	8 cells and that exogenous heparin competitively inhibits BMP-7 binding to endogenous HS.	bind
36921	2	8694	7	10	NULL	0	NULL	heparin	NULL	exogenous 	inhibits	NULL	competitively			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_308_4_858_s_170	12927798	8 cells and that exogenous heparin competitively inhibits BMP-7 binding to endogenous HS.	bind
37777	1	8696	5	13	NULL	NULL	NULL	Sp1	GP		is a type of					nuclear protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_907_s_22	12067897	8 DNase I footprinting analysis and electrophoretic mobility shift assay (EMSA) have demonstrated that Sp1 is the major nuclear protein binding to the Flk-1/KDR core promoter region.	bind
37778	2	8696	5	13	NULL	NULL	NULL	Sp1	GP		bind					Flk-1/KDR	GP			core promoter region	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_907_s_22	12067897	8 DNase I footprinting analysis and electrophoretic mobility shift assay (EMSA) have demonstrated that Sp1 is the major nuclear protein binding to the Flk-1/KDR core promoter region.	bind
36922	1	8696	7	NULL	NULL	0	NULL	 Sp1	NULL		bind	NULL				Flk-1/KDR	NULL			core promoter	NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_907_s_22	12067897	8 DNase I footprinting analysis and electrophoretic mobility shift assay (EMSA) have demonstrated that Sp1 is the major nuclear protein binding to the Flk-1/KDR core promoter region.	bind
36923	2	8696	7	NULL	NULL	0	NULL	Sp1	NULL		is a type of	NULL				nuclear binding protein	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_907_s_22	12067897	8 DNase I footprinting analysis and electrophoretic mobility shift assay (EMSA) have demonstrated that Sp1 is the major nuclear protein binding to the Flk-1/KDR core promoter region.	bind
37779	1	8697	5	13	NULL	NULL	NULL	FKBP12.6	GP		bind					RyR2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_4_487_s_25	14715536	8 Furthermore, a single mutation of serine-2808 to aspartate (S2808D) abolished FKBP12.6 binding to RyR2.	bind
37780	2	8697	5	13	NULL	NULL	NULL	FKBP12.6	GP	mutant	abolishes			S2808D		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_4_487_s_25	14715536	8 Furthermore, a single mutation of serine-2808 to aspartate (S2808D) abolished FKBP12.6 binding to RyR2.	bind
46721	3	8697	5	13	NULL	NULL	NULL	S2808D	AminoAcid		is					 serine-2808 to aspartate	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_4_487_s_25	14715536	8 Furthermore, a single mutation of serine-2808 to aspartate (S2808D) abolished FKBP12.6 binding to RyR2.	bind
36924	1	8697	7	NULL	NULL	0	NULL	FKBP12.6 	NULL		bind	NULL				RyR2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_4_487_s_25	14715536	8 Furthermore, a single mutation of serine-2808 to aspartate (S2808D) abolished FKBP12.6 binding to RyR2.	bind
36925	2	8697	7	NULL	NULL	0	NULL		NULL	mutant	abolish	NULL		S2808D		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_4_487_s_25	14715536	8 Furthermore, a single mutation of serine-2808 to aspartate (S2808D) abolished FKBP12.6 binding to RyR2.	bind
36926	3	8697	7	10	NULL	0	NULL	S2808D	NULL		is	NULL				serine-2808 to aspartate	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_4_487_s_25	14715536	8 Furthermore, a single mutation of serine-2808 to aspartate (S2808D) abolished FKBP12.6 binding to RyR2.	bind
37781	1	8698	5	13	NULL	NULL	NULL	PBEF	GP		bind					insulin receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_97_1_25_s_205	15947248	8 However, the physiological relevance of PBEF binding to the insulin receptor binding has been questioned.	bind
36927	1	8698	7	NULL	NULL	0	NULL	 PBEF	NULL		bind	NULL				insulin receptor	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_97_1_25_s_205	15947248	8 However, the physiological relevance of PBEF binding to the insulin receptor binding has been questioned.	bind
37782	1	8699	5	13	NULL	NULL	NULL	HSP90	GP		bind					hormone receptors	GP	intracellular			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1628_s_40	15231513	8 HSP90 binds intracellular hormone receptors.	bind
36928	1	8699	7	NULL	NULL	0	NULL	HSP90	NULL		binds	NULL				 hormone receptors	NULL	intracellular			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_9_1628_s_40	15231513	8 HSP90 binds intracellular hormone receptors.	bind
37783	1	8700	5	13	NULL	NULL	NULL	LPS	Chemical		associate with					lipoprotein classes	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2174_s_30	15388525	8 In the circulation, LPS associates with all lipoprotein classes, but it may promote atherogenesis when it invades the arterial wall complexed with LDL. 9,10  An LDL - LPS complex is recognized as minimally modified LDL, which readily binds to macrophage LPS receptors.	bind
37784	2	8700	5	13	NULL	NULL	NULL	arterial wall	OrganismPart		complex with					LDL	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2174_s_30	15388525	8 In the circulation, LPS associates with all lipoprotein classes, but it may promote atherogenesis when it invades the arterial wall complexed with LDL. 9,10  An LDL - LPS complex is recognized as minimally modified LDL, which readily binds to macrophage LPS receptors.	bind
37785	3	8700	5	13	NULL	NULL	NULL	statement 1	Process		occurs during					circulation	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2174_s_30	15388525	8 In the circulation, LPS associates with all lipoprotein classes, but it may promote atherogenesis when it invades the arterial wall complexed with LDL. 9,10  An LDL - LPS complex is recognized as minimally modified LDL, which readily binds to macrophage LPS receptors.	bind
37786	4	8700	5	13	NULL	NULL	NULL	LPS	Chemical		promotes					atherogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2174_s_30	15388525	8 In the circulation, LPS associates with all lipoprotein classes, but it may promote atherogenesis when it invades the arterial wall complexed with LDL. 9,10  An LDL - LPS complex is recognized as minimally modified LDL, which readily binds to macrophage LPS receptors.	bind
37787	5	8700	5	13	NULL	NULL	NULL	LPS	Chemical		invades					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2174_s_30	15388525	8 In the circulation, LPS associates with all lipoprotein classes, but it may promote atherogenesis when it invades the arterial wall complexed with LDL. 9,10  An LDL - LPS complex is recognized as minimally modified LDL, which readily binds to macrophage LPS receptors.	bind
37788	6	8700	5	13	NULL	NULL	NULL	statement 5	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2174_s_30	15388525	8 In the circulation, LPS associates with all lipoprotein classes, but it may promote atherogenesis when it invades the arterial wall complexed with LDL. 9,10  An LDL - LPS complex is recognized as minimally modified LDL, which readily binds to macrophage LPS receptors.	bind
37789	7	8700	5	13	NULL	NULL	NULL	LDL - LPS complex	GP		is recognized as					LDL	GP	minimally modified			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2174_s_30	15388525	8 In the circulation, LPS associates with all lipoprotein classes, but it may promote atherogenesis when it invades the arterial wall complexed with LDL. 9,10  An LDL - LPS complex is recognized as minimally modified LDL, which readily binds to macrophage LPS receptors.	bind
37790	8	8700	5	13	NULL	NULL	NULL	statement 7	Process		bind		readily			LPS receptors	GP	macrophage			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2174_s_30	15388525	8 In the circulation, LPS associates with all lipoprotein classes, but it may promote atherogenesis when it invades the arterial wall complexed with LDL. 9,10  An LDL - LPS complex is recognized as minimally modified LDL, which readily binds to macrophage LPS receptors.	bind
37791	9	8700	5	13	NULL	NULL	NULL	statement 4	Process		occurs during					circulation	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2174_s_30	15388525	8 In the circulation, LPS associates with all lipoprotein classes, but it may promote atherogenesis when it invades the arterial wall complexed with LDL. 9,10  An LDL - LPS complex is recognized as minimally modified LDL, which readily binds to macrophage LPS receptors.	bind
36929	1	8700	7	NULL	NULL	0	NULL	LPS	NULL		associate with	NULL				lipoproteins	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2174_s_30	15388525	8 In the circulation, LPS associates with all lipoprotein classes, but it may promote atherogenesis when it invades the arterial wall complexed with LDL. 9,10  An LDL - LPS complex is recognized as minimally modified LDL, which readily binds to macrophage LPS receptors.	bind
36930	2	8700	7	NULL	NULL	0	NULL	LPS	NULL		complex with	NULL				LDL	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2174_s_30	15388525	8 In the circulation, LPS associates with all lipoprotein classes, but it may promote atherogenesis when it invades the arterial wall complexed with LDL. 9,10  An LDL - LPS complex is recognized as minimally modified LDL, which readily binds to macrophage LPS receptors.	bind
36931	3	8700	7	NULL	NULL	0	NULL	statement 2	NULL		promote	NULL	may			atherogenesis	NULL				NULL	arterial wall	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2174_s_30	15388525	8 In the circulation, LPS associates with all lipoprotein classes, but it may promote atherogenesis when it invades the arterial wall complexed with LDL. 9,10  An LDL - LPS complex is recognized as minimally modified LDL, which readily binds to macrophage LPS receptors.	bind
36932	4	8700	7	NULL	NULL	0	NULL	LDL-LPS	NULL		binds to	NULL				LPS receptors	NULL	macrophage			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2174_s_30	15388525	8 In the circulation, LPS associates with all lipoprotein classes, but it may promote atherogenesis when it invades the arterial wall complexed with LDL. 9,10  An LDL - LPS complex is recognized as minimally modified LDL, which readily binds to macrophage LPS receptors.	bind
36933	5	8700	7	NULL	NULL	0	NULL	LDL-LPS complex	NULL		is recognized as	NULL				LDL	NULL	minimally modified			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2174_s_30	15388525	8 In the circulation, LPS associates with all lipoprotein classes, but it may promote atherogenesis when it invades the arterial wall complexed with LDL. 9,10  An LDL - LPS complex is recognized as minimally modified LDL, which readily binds to macrophage LPS receptors.	bind
37792	1	8701	5	13	NULL	NULL	NULL	SR	CellComponent		bind					FKBP12.6	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_107_3_477_s_104	12551874	8 Note that the MCA fluorescence (net value, in arbitrary units: labeled SR minus unlabeled  SR) increased as SR became FKBP12.6-deficient but decreased as SR bound FKBP12.6  again.	bind
36934	1	8701	7	NULL	NULL	0	NULL	SR	NULL		bind	NULL				FKBP12.6	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_107_3_477_s_104	12551874	8 Note that the MCA fluorescence (net value, in arbitrary units: labeled SR minus unlabeled  SR) increased as SR became FKBP12.6-deficient but decreased as SR bound FKBP12.6  again.	bind
37793	1	8703	5	13	NULL	NULL	NULL	VDR	GP		bind					RXR(s)	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_269_4_8300629_s_11	8300629	8 nuclear extracts suggest  that the VDR binds to the mouse osteopontin VDRE predominantly as a heterodimer  with retinoid X receptor(s) (RXR(s)).	bind
37794	2	8703	5	13	NULL	NULL	NULL	RXR(s)	GP		is					retinoid X receptor(s)	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_269_4_8300629_s_11	8300629	8 nuclear extracts suggest  that the VDR binds to the mouse osteopontin VDRE predominantly as a heterodimer  with retinoid X receptor(s) (RXR(s)).	bind
37795	3	8703	5	13	NULL	NULL	NULL	statement 1	GP		forms					VDR-RXR(s) heterodimer	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_269_4_8300629_s_11	8300629	8 nuclear extracts suggest  that the VDR binds to the mouse osteopontin VDRE predominantly as a heterodimer  with retinoid X receptor(s) (RXR(s)).	bind
37796	4	8703	5	13	NULL	NULL	NULL	VDR-RXR(s) heterodimer	GP		bind					osteopontin	GP	mouse		VDRE	NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_269_4_8300629_s_11	8300629	8 nuclear extracts suggest  that the VDR binds to the mouse osteopontin VDRE predominantly as a heterodimer  with retinoid X receptor(s) (RXR(s)).	bind
36938	1	8703	7	NULL	NULL	0	NULL	VDR	NULL		heterodimerizes with	NULL				RXR	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_269_4_8300629_s_11	8300629	8 nuclear extracts suggest  that the VDR binds to the mouse osteopontin VDRE predominantly as a heterodimer  with retinoid X receptor(s) (RXR(s)).	bind
36939	2	8703	7	10	NULL	0	NULL	statement 1			binds to					osteopontin		mouse		VDRE	NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_269_4_8300629_s_11	8300629	8 nuclear extracts suggest  that the VDR binds to the mouse osteopontin VDRE predominantly as a heterodimer  with retinoid X receptor(s) (RXR(s)).	bind
36940	3	8703	7	NULL	NULL	0	NULL	RXR	NULL		is	NULL				retinoid X receptor	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_269_4_8300629_s_11	8300629	8 nuclear extracts suggest  that the VDR binds to the mouse osteopontin VDRE predominantly as a heterodimer  with retinoid X receptor(s) (RXR(s)).	bind
37798	1	8704	5	13	NULL	NULL	NULL	PDGF-A	GP		bind					PDGFR-alpha	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_5_479_s_22	15297375	8 Of the 2 high-affinity PDGF receptors (PDGFRs), PDGF-A binds to PDGFR-alpha but not receptor-beta.	bind
37799	2	8704	5	13	NULL	NULL	NULL	PDGF-A	GP		does not bind					PDGFR-beta	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_5_479_s_22	15297375	8 Of the 2 high-affinity PDGF receptors (PDGFRs), PDGF-A binds to PDGFR-alpha but not receptor-beta.	bind
37800	3	8704	5	13	NULL	NULL	NULL	PDGFR-alpha	GP		is a type of					PDGF receptors	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_5_479_s_22	15297375	8 Of the 2 high-affinity PDGF receptors (PDGFRs), PDGF-A binds to PDGFR-alpha but not receptor-beta.	bind
37801	4	8704	5	13	NULL	NULL	NULL	PDGFR-beta	GP		is a type of					PDGF receptors	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_5_479_s_22	15297375	8 Of the 2 high-affinity PDGF receptors (PDGFRs), PDGF-A binds to PDGFR-alpha but not receptor-beta.	bind
36941	1	8704	7	NULL	NULL	0	NULL	PDGF-A	NULL		bind	NULL				PDGFR-alpha	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_95_5_479_s_22	15297375	8 Of the 2 high-affinity PDGF receptors (PDGFRs), PDGF-A binds to PDGFR-alpha but not receptor-beta.	bind
36943	2	8704	7	NULL	NULL	0	NULL	PDGF-A 	NULL		does not bind	NULL				PDGFR-beta	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_95_5_479_s_22	15297375	8 Of the 2 high-affinity PDGF receptors (PDGFRs), PDGF-A binds to PDGFR-alpha but not receptor-beta.	bind
36944	3	8704	7	10	NULL	0	NULL	PDGFR	NULL		is a type of 	NULL				PDGF receptor	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_5_479_s_22	15297375	8 Of the 2 high-affinity PDGF receptors (PDGFRs), PDGF-A binds to PDGFR-alpha but not receptor-beta.	bind
37802	1	8705	5	13	NULL	NULL	NULL	cytochrome c	GP		bind					CcP	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1597_2_193_s_1550	12044899	8 The reaction of CcP and hydrogen peroxide is not inhibited by binding of cytochrome  c to CcP [  159].	bind
37803	2	8705	5	13	NULL	NULL	NULL	CcP	GP	reaction of	is not inhibited by					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1597_2_193_s_1550	12044899	8 The reaction of CcP and hydrogen peroxide is not inhibited by binding of cytochrome  c to CcP [  159].	bind
37804	3	8705	5	13	NULL	NULL	NULL	hydrogen peroxide	Chemical	reaction of	is not inhibited by					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1597_2_193_s_1550	12044899	8 The reaction of CcP and hydrogen peroxide is not inhibited by binding of cytochrome  c to CcP [  159].	bind
36945	1	8705	7	NULL	NULL	0	NULL	cytochrome c 	NULL		bind	NULL				CcP	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1597_2_193_s_1550	12044899	8 The reaction of CcP and hydrogen peroxide is not inhibited by binding of cytochrome  c to CcP [  159].	bind
36946	2	8705	7	NULL	NULL	0	NULL	statement 1	NULL		does not inhibit	NULL				CcP	NULL	reaction of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1597_2_193_s_1550	12044899	8 The reaction of CcP and hydrogen peroxide is not inhibited by binding of cytochrome  c to CcP [  159].	bind
36947	3	8705	7	NULL	NULL	0	NULL	statement 1	NULL		does not inhibit	NULL				hydrogen peroxide	NULL	reaction of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1597_2_193_s_1550	12044899	8 The reaction of CcP and hydrogen peroxide is not inhibited by binding of cytochrome  c to CcP [  159].	bind
37805	1	8706	5	13	NULL	NULL	NULL	KLF5	GP		bind					PDGF-A	GP	endogenous		promoter	NULL	SMCs	NULL	NULL	NULL	NULL	gw70_circulationres_97_11_1132_s_147	16224062	8 The results showed that KLF5, RARalpha, and RXRalpha all bound to the endogenous  PDGF-A promoter in SMCs and that Am80 markedly reduced the abundance of the  PDGF-A promoter sequence in the immunoprecipitates pulled down with anti-KLF5, anti-RARalpha, or anti-RXRalpha antibody.	bind
37806	2	8706	5	13	NULL	NULL	NULL	RARalpha	GP		bind					PDGF-A	GP	endogenous		promoter	NULL	SMCs	NULL	NULL	NULL	NULL	gw70_circulationres_97_11_1132_s_147	16224062	8 The results showed that KLF5, RARalpha, and RXRalpha all bound to the endogenous  PDGF-A promoter in SMCs and that Am80 markedly reduced the abundance of the  PDGF-A promoter sequence in the immunoprecipitates pulled down with anti-KLF5, anti-RARalpha, or anti-RXRalpha antibody.	bind
37807	3	8706	5	13	NULL	NULL	NULL	RXRalpha	GP		bind					PDGF-A	GP	endogenous		promoter	NULL	SMCs	NULL	NULL	NULL	NULL	gw70_circulationres_97_11_1132_s_147	16224062	8 The results showed that KLF5, RARalpha, and RXRalpha all bound to the endogenous  PDGF-A promoter in SMCs and that Am80 markedly reduced the abundance of the  PDGF-A promoter sequence in the immunoprecipitates pulled down with anti-KLF5, anti-RARalpha, or anti-RXRalpha antibody.	bind
36951	1	8706	7	NULL	NULL	0	NULL	 KLF5	NULL		bind	NULL				PDGF-A	NULL	endogenous		promoter	NULL	SMCs	0	NULL	NULL	NULL	gw70_circulationres_97_11_1132_s_147	16224062	8 The results showed that KLF5, RARalpha, and RXRalpha all bound to the endogenous  PDGF-A promoter in SMCs and that Am80 markedly reduced the abundance of the  PDGF-A promoter sequence in the immunoprecipitates pulled down with anti-KLF5, anti-RARalpha, or anti-RXRalpha antibody.	bind
36952	2	8706	7	NULL	NULL	0	NULL	RARalpha	NULL		bind	NULL				PDGF-A	NULL	endogenous		promoter	NULL	SMCs	NULL	NULL	NULL	NULL	gw70_circulationres_97_11_1132_s_147	16224062	8 The results showed that KLF5, RARalpha, and RXRalpha all bound to the endogenous  PDGF-A promoter in SMCs and that Am80 markedly reduced the abundance of the  PDGF-A promoter sequence in the immunoprecipitates pulled down with anti-KLF5, anti-RARalpha, or anti-RXRalpha antibody.	bind
36953	3	8706	7	NULL	NULL	0	NULL	 RXRalpha	NULL		bind	NULL				PDGF-A	NULL	endogenous		promoter	NULL	SMcs	0	NULL	NULL	NULL	gw70_circulationres_97_11_1132_s_147	16224062	8 The results showed that KLF5, RARalpha, and RXRalpha all bound to the endogenous  PDGF-A promoter in SMCs and that Am80 markedly reduced the abundance of the  PDGF-A promoter sequence in the immunoprecipitates pulled down with anti-KLF5, anti-RARalpha, or anti-RXRalpha antibody.	bind
37811	1	8707	5	13	NULL	NULL	NULL	ATP	Chemical		bind					ArsA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_23_16153_s_336	10347168	8 The second-order association rate constant ( k1) for the binding of ATP to ArsA was calculated from the measured  Kd and the apparent rate of dissociation.	bind
36954	1	8707	7	NULL	NULL	0	NULL	 ATP	NULL		bind	NULL				ArsA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_23_16153_s_336	10347168	8 The second-order association rate constant ( k1) for the binding of ATP to ArsA was calculated from the measured  Kd and the apparent rate of dissociation.	bind
38745	1	8708	5	13	NULL	NULL	NULL	NOS3	GP	stimulated	does not bind					calmodulin	GP				NULL	oxLDL-treated cells	NULL	NULL	NULL	NULL	gw70_circulationres_98_6_717_s_63	16574911	8 These authors found that NOS3 from the oxLDL-treated cells no longer bound calmodulin when stimulated, and that NOS3 was less prominently associated with the Golgi and plasma membranes resulting in cytosolic NOS3 distribution.	bind
38746	2	8708	5	13	NULL	NULL	NULL	NOS3	GP		associate with		less prominently			Golgi	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_717_s_63	16574911	8 These authors found that NOS3 from the oxLDL-treated cells no longer bound calmodulin when stimulated, and that NOS3 was less prominently associated with the Golgi and plasma membranes resulting in cytosolic NOS3 distribution.	bind
38747	3	8708	5	13	NULL	NULL	NULL	NOS3	GP		associate with		less prominently			plasma membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_717_s_63	16574911	8 These authors found that NOS3 from the oxLDL-treated cells no longer bound calmodulin when stimulated, and that NOS3 was less prominently associated with the Golgi and plasma membranes resulting in cytosolic NOS3 distribution.	bind
38748	4	8708	5	13	NULL	NULL	NULL	statement 2	Process		results in					NOS3	GP	distribution of;;cytosolic			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_717_s_63	16574911	8 These authors found that NOS3 from the oxLDL-treated cells no longer bound calmodulin when stimulated, and that NOS3 was less prominently associated with the Golgi and plasma membranes resulting in cytosolic NOS3 distribution.	bind
38749	5	8708	5	13	NULL	NULL	NULL	statement 3	Process		results in					NOS3	GP	distribution of;;cytosolic			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_717_s_63	16574911	8 These authors found that NOS3 from the oxLDL-treated cells no longer bound calmodulin when stimulated, and that NOS3 was less prominently associated with the Golgi and plasma membranes resulting in cytosolic NOS3 distribution.	bind
36955	1	8708	7	10	NULL	0	NULL	NOS3 		stimulated	does not bind					calmodulin 					NULL	oxLDL-treated cells	NULL	NULL	NULL	NULL	gw70_circulationres_98_6_717_s_63	16574911	8 These authors found that NOS3 from the oxLDL-treated cells no longer bound calmodulin when stimulated, and that NOS3 was less prominently associated with the Golgi and plasma membranes resulting in cytosolic NOS3 distribution.	bind
36956	2	8708	7	NULL	NULL	0	NULL	NOS3	NULL		associate with	NULL				golgi membrane	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_6_717_s_63	16574911	8 These authors found that NOS3 from the oxLDL-treated cells no longer bound calmodulin when stimulated, and that NOS3 was less prominently associated with the Golgi and plasma membranes resulting in cytosolic NOS3 distribution.	bind
36957	3	8708	7	NULL	NULL	0	NULL	NOS3	NULL		associate with	NULL				plasma membrane	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_6_717_s_63	16574911	8 These authors found that NOS3 from the oxLDL-treated cells no longer bound calmodulin when stimulated, and that NOS3 was less prominently associated with the Golgi and plasma membranes resulting in cytosolic NOS3 distribution.	bind
36958	4	8708	7	10	NULL	0	NULL	statement 2	NULL		result in	NULL				NOS3	NULL	cytosolic;; distribution of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_717_s_63	16574911	8 These authors found that NOS3 from the oxLDL-treated cells no longer bound calmodulin when stimulated, and that NOS3 was less prominently associated with the Golgi and plasma membranes resulting in cytosolic NOS3 distribution.	bind
36959	5	8708	7	10	NULL	0	NULL	statement 3	NULL		result in	NULL				NOS3	NULL	cytosolic;; distribution of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_6_717_s_63	16574911	8 These authors found that NOS3 from the oxLDL-treated cells no longer bound calmodulin when stimulated, and that NOS3 was less prominently associated with the Golgi and plasma membranes resulting in cytosolic NOS3 distribution.	bind
37812	1	8709	5	13	NULL	NULL	NULL	CCR2	GP		is					CC type chemokine receptor 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_12_1436_s_163	11560862	8, 24 The CC type chemokine receptor 2 (CCR2), which binds to MCP-1, is necessary for the development of Ang II-induced macrophage infiltration and vascular hypertrophy.	bind
37813	2	8709	5	13	NULL	NULL	NULL	CCR2	GP		bind					MCP-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_12_1436_s_163	11560862	8, 24 The CC type chemokine receptor 2 (CCR2), which binds to MCP-1, is necessary for the development of Ang II-induced macrophage infiltration and vascular hypertrophy.	bind
37814	3	8709	5	13	NULL	NULL	NULL	Ang II	GP		induce					macrophage infiltration	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_12_1436_s_163	11560862	8, 24 The CC type chemokine receptor 2 (CCR2), which binds to MCP-1, is necessary for the development of Ang II-induced macrophage infiltration and vascular hypertrophy.	bind
37815	4	8709	5	13	NULL	NULL	NULL	Ang II	GP		induce					vascular hypertrophy	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_12_1436_s_163	11560862	8, 24 The CC type chemokine receptor 2 (CCR2), which binds to MCP-1, is necessary for the development of Ang II-induced macrophage infiltration and vascular hypertrophy.	bind
37816	5	8709	5	13	NULL	NULL	NULL	statement 2	Process		is necessary for					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_12_1436_s_163	11560862	8, 24 The CC type chemokine receptor 2 (CCR2), which binds to MCP-1, is necessary for the development of Ang II-induced macrophage infiltration and vascular hypertrophy.	bind
37817	6	8709	5	13	NULL	NULL	NULL	statement 3	Process		is necessary for					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_104_12_1436_s_163	11560862	8, 24 The CC type chemokine receptor 2 (CCR2), which binds to MCP-1, is necessary for the development of Ang II-induced macrophage infiltration and vascular hypertrophy.	bind
36961	1	8709	7	NULL	NULL	0	NULL	CCR2	NULL		binds to	NULL				MCP-1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_104_12_1436_s_163	11560862	8, 24 The CC type chemokine receptor 2 (CCR2), which binds to MCP-1, is necessary for the development of Ang II-induced macrophage infiltration and vascular hypertrophy.	bind
36962	2	8709	7	NULL	NULL	0	NULL	CCR2	NULL		is	NULL				CC type chemokine receptor 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_104_12_1436_s_163	11560862	8, 24 The CC type chemokine receptor 2 (CCR2), which binds to MCP-1, is necessary for the development of Ang II-induced macrophage infiltration and vascular hypertrophy.	bind
36963	3	8709	7	NULL	NULL	0	NULL	Ang II 	NULL		induce	NULL				macrophage infiltration	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_104_12_1436_s_163	11560862	8, 24 The CC type chemokine receptor 2 (CCR2), which binds to MCP-1, is necessary for the development of Ang II-induced macrophage infiltration and vascular hypertrophy.	bind
36964	4	8709	7	NULL	NULL	0	NULL	Ang II 	NULL		induce	NULL				vascular hypertrophy	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_104_12_1436_s_163	11560862	8, 24 The CC type chemokine receptor 2 (CCR2), which binds to MCP-1, is necessary for the development of Ang II-induced macrophage infiltration and vascular hypertrophy.	bind
36965	5	8709	7	NULL	NULL	0	NULL	statement 1	NULL		is necessary for	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_104_12_1436_s_163	11560862	8, 24 The CC type chemokine receptor 2 (CCR2), which binds to MCP-1, is necessary for the development of Ang II-induced macrophage infiltration and vascular hypertrophy.	bind
36966	6	8709	7	NULL	NULL	0	NULL	statement 1	NULL		is necessary for	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_104_12_1436_s_163	11560862	8, 24 The CC type chemokine receptor 2 (CCR2), which binds to MCP-1, is necessary for the development of Ang II-induced macrophage infiltration and vascular hypertrophy.	bind
37937	1	8710	5	13	NULL	NULL	NULL				bind		noncovalently	carboxy-terminal	4-kDa carboxy-terminal fragment of 36 residues (C-36)	complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_11_1801_s_22	11701469	8, 9 The resulting 4-kDa carboxy-terminal fragment of 36 residues (C-36) still binds the complex noncovalently, but under denaturing conditions in vitro, the C-36 fragment dissociates from the complex.	bind
37938	2	8710	5	13	NULL	NULL	NULL				dissociates from			C-36 fragment		complex	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_11_1801_s_22	11701469	8, 9 The resulting 4-kDa carboxy-terminal fragment of 36 residues (C-36) still binds the complex noncovalently, but under denaturing conditions in vitro, the C-36 fragment dissociates from the complex.	bind
37939	3	8710	5	13	NULL	NULL	NULL	statement 2	Process		occurs under					denaturing conditions					NULL	in vitro	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_11_1801_s_22	11701469	8, 9 The resulting 4-kDa carboxy-terminal fragment of 36 residues (C-36) still binds the complex noncovalently, but under denaturing conditions in vitro, the C-36 fragment dissociates from the complex.	bind
37909	1	8710	7	NULL	NULL	0	NULL		NULL		binds	NULL	noncovalently	4-kDa carboxy-terminal fragment of 36 residues (C-36)		complex	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_11_1801_s_22	11701469	8, 9 The resulting 4-kDa carboxy-terminal fragment of 36 residues (C-36) still binds the complex noncovalently, but under denaturing conditions in vitro, the C-36 fragment dissociates from the complex.	bind
37910	2	8710	7	NULL	NULL	0	NULL		NULL		dissociates from	NULL		C-36 fragment		complex	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_11_1801_s_22	11701469	8, 9 The resulting 4-kDa carboxy-terminal fragment of 36 residues (C-36) still binds the complex noncovalently, but under denaturing conditions in vitro, the C-36 fragment dissociates from the complex.	bind
37911	3	8710	7	NULL	NULL	0	NULL	statement 2	NULL		occurs under	NULL				denaturing condition	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_11_1801_s_22	11701469	8, 9 The resulting 4-kDa carboxy-terminal fragment of 36 residues (C-36) still binds the complex noncovalently, but under denaturing conditions in vitro, the C-36 fragment dissociates from the complex.	bind
37818	1	8711	5	13	NULL	NULL	NULL	MPO	GP		bind					vessel wall	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_circulation_113_15_1871_s_84	16606792	8,10  To test whether heparins also reverse MPO binding to the vessel wall, isolated extracellular matrix proteins, cultured endothelial cells, and saphenous vein graft specimens from patients undergoing aortocoronary bypass surgery were analyzed for MPO before and after treatment with heparin.	bind
36967	1	8711	7	NULL	NULL	0	NULL	MPO	NULL		bind	NULL				vessel wall	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_113_15_1871_s_84	16606792	8,10  To test whether heparins also reverse MPO binding to the vessel wall, isolated extracellular matrix proteins, cultured endothelial cells, and saphenous vein graft specimens from patients undergoing aortocoronary bypass surgery were analyzed for MPO before and after treatment with heparin.	bind
37819	1	8712	5	13	NULL	NULL	NULL	Ang2	GP		bind					Tie2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_11_1373_s_31	16690881	8,26  Ang2 binds to Tie2 and acts as a competing Ang1 antagonist but can also phosphorylate Tie2.	bind
37822	2	8712	5	13	NULL	NULL	NULL	Ang2	GP		acts as a					Ang1 antagonist	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_11_1373_s_31	16690881	8,26  Ang2 binds to Tie2 and acts as a competing Ang1 antagonist but can also phosphorylate Tie2.	bind
37823	3	8712	5	13	NULL	NULL	NULL	Ang2	GP		phosphorylate					Tie2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_11_1373_s_31	16690881	8,26  Ang2 binds to Tie2 and acts as a competing Ang1 antagonist but can also phosphorylate Tie2.	bind
36975	1	8712	7	NULL	NULL	0	NULL	Ang2	NULL		binds to	NULL				Tie2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_11_1373_s_31	16690881	8,26  Ang2 binds to Tie2 and acts as a competing Ang1 antagonist but can also phosphorylate Tie2.	bind
36976	2	8712	7	NULL	NULL	0	NULL	Ang2	NULL		acts as a	NULL				Ang1 antagonist	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_11_1373_s_31	16690881	8,26  Ang2 binds to Tie2 and acts as a competing Ang1 antagonist but can also phosphorylate Tie2.	bind
36977	3	8712	7	NULL	NULL	0	NULL	Ang2	NULL		phosphorylate	NULL				Tie2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_11_1373_s_31	16690881	8,26  Ang2 binds to Tie2 and acts as a competing Ang1 antagonist but can also phosphorylate Tie2.	bind
56311	1	8713	5	13	NULL	NULL	NULL	cAMP	Chemical		bind					52 kDa protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_37_8_1081_s_92	9833637	8- N3-[32]cAMP binding to the 52 kDa protein band (indicated by arrow) in microtubules	bind
36978	1	8713	7	10	NULL	0	NULL	cAMP			bind					52 kDa protein 					NULL	microtubules	NULL	NULL	NULL	NULL	gw60_neuropharmacology_37_8_1081_s_92	9833637	8- N3-[32]cAMP binding to the 52 kDa protein band (indicated by arrow) in microtubules	bind
37824	1	8714	5	13	NULL	NULL	NULL	ANS	Chemical		bind					N-PLA2	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_453_3_395_s_36	10405184	8-Anilino-1-naphthalene sulfonate (ANS) was included in the N-PLA2 containing solution to monitor the possible heparin-induced fluorescence changes of the ANS bound to N-PLA2.	bind
46753	2	8714	5	13	NULL	NULL	NULL	ANS	Chemical		is					8-Anilino-1-naphthalene sulfonate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_453_3_395_s_36	10405184	8-Anilino-1-naphthalene sulfonate (ANS) was included in the N-PLA2 containing solution to monitor the possible heparin-induced fluorescence changes of the ANS bound to N-PLA2.	bind
36979	1	8714	7	NULL	NULL	0	NULL	ANS 	NULL		bind	NULL				N-PLA2	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_453_3_395_s_36	10405184	8-Anilino-1-naphthalene sulfonate (ANS) was included in the N-PLA2 containing solution to monitor the possible heparin-induced fluorescence changes of the ANS bound to N-PLA2.	bind
36980	2	8714	7	NULL	NULL	0	NULL	ANS	NULL		is	NULL				8-Anilino-1-naphthalene sulfonate	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_453_3_395_s_36	10405184	8-Anilino-1-naphthalene sulfonate (ANS) was included in the N-PLA2 containing solution to monitor the possible heparin-induced fluorescence changes of the ANS bound to N-PLA2.	bind
37825	1	8716	5	13	NULL	NULL	NULL	8-Azido-ATP	Chemical		bind					ABCG1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_47_8_1791_s_173	16702602	8-Azido-ATP binding of ABCG1.	bind
36984	1	8716	7	NULL	NULL	0	NULL	8-Azido-ATP	NULL		bind	NULL				ABCG1	NULL				NULL		0	NULL	NULL	NULL	gw70_jlipidres_47_8_1791_s_173	16702602	8-Azido-ATP binding of ABCG1.	bind
37826	1	8717	5	13	NULL	NULL	NULL	8-Azido-ATP	Chemical		bind							mutant	C431A		NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1461_2_305_s_157	10581363	8-Azido-ATP binding of the C431A mutant form appeared not to be affected by treatment with 100  M NEM.	bind
36985	1	8717	7	NULL	NULL	0	NULL	8-Azido-ATP	NULL		bind	NULL					NULL	mutant	C431A		NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1461_2_305_s_157	10581363	8-Azido-ATP binding of the C431A mutant form appeared not to be affected by treatment with 100  M NEM.	bind
37828	1	8718	5	13	NULL	NULL	NULL	8-Azido-ATP	Chemical		bind					SURx	GP		NBF1		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_37_28757_s_84	10893240	8-Azido-ATP Binding to NBF1 and NBF2 of SURx-- To investigate the ATP-binding properties of NBFs of SURx, SURx was photoaffinity-labeled with 50 muM 8-azido-[alpha-32]ATP under various conditions and mildly digested with trypsin (Fig.  3).	bind
37829	2	8718	5	13	NULL	NULL	NULL	8-Azido-ATP	Chemical		bind					SURx	GP		NBF2		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_37_28757_s_84	10893240	8-Azido-ATP Binding to NBF1 and NBF2 of SURx-- To investigate the ATP-binding properties of NBFs of SURx, SURx was photoaffinity-labeled with 50 muM 8-azido-[alpha-32]ATP under various conditions and mildly digested with trypsin (Fig.  3).	bind
36986	1	8718	7	10	NULL	0	NULL	8-azido-[alpha-32]ATP	NULL		bind	NULL				SURx	NULL		NBF1		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_37_28757_s_84	10893240	8-Azido-ATP Binding to NBF1 and NBF2 of SURx-- To investigate the ATP-binding properties of NBFs of SURx, SURx was photoaffinity-labeled with 50 muM 8-azido-[alpha-32]ATP under various conditions and mildly digested with trypsin (Fig.  3).	bind
36987	2	8718	7	10	NULL	0	NULL	 8-azido-[alpha-32]ATP	NULL		bind	NULL				SURx	NULL		NBF2		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_37_28757_s_84	10893240	8-Azido-ATP Binding to NBF1 and NBF2 of SURx-- To investigate the ATP-binding properties of NBFs of SURx, SURx was photoaffinity-labeled with 50 muM 8-azido-[alpha-32]ATP under various conditions and mildly digested with trypsin (Fig.  3).	bind
37830	1	8719	5	13	NULL	NULL	NULL	8-Azido-ATP	Chemical		bind					TAP1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_32_29686_s_129	12777379	8-Azido-ATP Binding to TAP1 and TAP2 Is Magnesium- and  Temperature-dependent -- Magnesium is well known to be required for  ATP hydrolysis by most ATPases.	bind
37831	2	8719	5	13	NULL	NULL	NULL	statement 1	Process		is dependent on					magnesium	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_32_29686_s_129	12777379	8-Azido-ATP Binding to TAP1 and TAP2 Is Magnesium- and  Temperature-dependent -- Magnesium is well known to be required for  ATP hydrolysis by most ATPases.	bind
37832	3	8719	5	13	NULL	NULL	NULL	statement 1	Process		is dependent on					temperature					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_32_29686_s_129	12777379	8-Azido-ATP Binding to TAP1 and TAP2 Is Magnesium- and  Temperature-dependent -- Magnesium is well known to be required for  ATP hydrolysis by most ATPases.	bind
37833	4	8719	5	13	NULL	NULL	NULL	8-Azido-ATP	Chemical		bind					TAP2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_32_29686_s_129	12777379	8-Azido-ATP Binding to TAP1 and TAP2 Is Magnesium- and  Temperature-dependent -- Magnesium is well known to be required for  ATP hydrolysis by most ATPases.	bind
37834	5	8719	5	13	NULL	NULL	NULL	statement 4	Process		is dependent on					magnesium	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_32_29686_s_129	12777379	8-Azido-ATP Binding to TAP1 and TAP2 Is Magnesium- and  Temperature-dependent -- Magnesium is well known to be required for  ATP hydrolysis by most ATPases.	bind
37835	6	8719	5	13	NULL	NULL	NULL	statement 4	Process		is dependent on					temperature					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_32_29686_s_129	12777379	8-Azido-ATP Binding to TAP1 and TAP2 Is Magnesium- and  Temperature-dependent -- Magnesium is well known to be required for  ATP hydrolysis by most ATPases.	bind
56312	7	8719	5	13	NULL	NULL	NULL	ATPase	GP		hydrolyse					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_32_29686_s_129	12777379	8-Azido-ATP Binding to TAP1 and TAP2 Is Magnesium- and  Temperature-dependent -- Magnesium is well known to be required for  ATP hydrolysis by most ATPases.	bind
56313	8	8719	5	13	NULL	NULL	NULL	magnesium	Chemical		ia required for					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_32_29686_s_129	12777379	8-Azido-ATP Binding to TAP1 and TAP2 Is Magnesium- and  Temperature-dependent -- Magnesium is well known to be required for  ATP hydrolysis by most ATPases.	bind
36988	1	8719	7	NULL	NULL	0	NULL	8-Azido-ATP	NULL		bind	NULL				TAP1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_32_29686_s_129	12777379	8-Azido-ATP Binding to TAP1 and TAP2 Is Magnesium- and  Temperature-dependent -- Magnesium is well known to be required for  ATP hydrolysis by most ATPases.	bind
36989	2	8719	7	NULL	NULL	0	NULL	8-Azido-ATP	NULL		bind	NULL				TAP2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_32_29686_s_129	12777379	8-Azido-ATP Binding to TAP1 and TAP2 Is Magnesium- and  Temperature-dependent -- Magnesium is well known to be required for  ATP hydrolysis by most ATPases.	bind
36990	3	8719	7	NULL	NULL	0	NULL	statement 1	NULL		depends on	NULL				Magnesium	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_32_29686_s_129	12777379	8-Azido-ATP Binding to TAP1 and TAP2 Is Magnesium- and  Temperature-dependent -- Magnesium is well known to be required for  ATP hydrolysis by most ATPases.	bind
36991	4	8719	7	NULL	NULL	0	NULL	statement 2	NULL		depends on	NULL				Magnesium	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_32_29686_s_129	12777379	8-Azido-ATP Binding to TAP1 and TAP2 Is Magnesium- and  Temperature-dependent -- Magnesium is well known to be required for  ATP hydrolysis by most ATPases.	bind
36992	5	8719	7	NULL	NULL	0	NULL	statement 1	NULL		depends on	NULL				temperature	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_32_29686_s_129	12777379	8-Azido-ATP Binding to TAP1 and TAP2 Is Magnesium- and  Temperature-dependent -- Magnesium is well known to be required for  ATP hydrolysis by most ATPases.	bind
36993	6	8719	7	NULL	NULL	0	NULL	statement 2	NULL		depends on	NULL				temperature	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_32_29686_s_129	12777379	8-Azido-ATP Binding to TAP1 and TAP2 Is Magnesium- and  Temperature-dependent -- Magnesium is well known to be required for  ATP hydrolysis by most ATPases.	bind
36994	7	8719	7	NULL	NULL	0	NULL	ATPases	NULL		hydrolyse	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_32_29686_s_129	12777379	8-Azido-ATP Binding to TAP1 and TAP2 Is Magnesium- and  Temperature-dependent -- Magnesium is well known to be required for  ATP hydrolysis by most ATPases.	bind
36995	8	8719	7	NULL	NULL	0	NULL	Magnesium	NULL		is required for	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_32_29686_s_129	12777379	8-Azido-ATP Binding to TAP1 and TAP2 Is Magnesium- and  Temperature-dependent -- Magnesium is well known to be required for  ATP hydrolysis by most ATPases.	bind
37836	1	8720	5	13	NULL	NULL	NULL	8-Azido-ATP	Chemical		bind					MDR1	GP	wild-type			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1461_2_305_s_156	10581363	8-Azido-ATP binding with the wild-type MDR1 was inhibited by 100  M NEM, while 8-azido-ATP binding with the C431A/C1074A mutant form was not, suggesting that the cysteines of Walker A motifs in both NBFs are responsible for the effects of NEM on ATP binding.	bind
37837	2	8720	5	13	NULL	NULL	NULL	NEM	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1461_2_305_s_156	10581363	8-Azido-ATP binding with the wild-type MDR1 was inhibited by 100  M NEM, while 8-azido-ATP binding with the C431A/C1074A mutant form was not, suggesting that the cysteines of Walker A motifs in both NBFs are responsible for the effects of NEM on ATP binding.	bind
37838	3	8720	5	13	NULL	NULL	NULL	8-azido-ATP	Chemical		bind					MDR1	GP	mutant	C431A;;C1074A		NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1461_2_305_s_156	10581363	8-Azido-ATP binding with the wild-type MDR1 was inhibited by 100  M NEM, while 8-azido-ATP binding with the C431A/C1074A mutant form was not, suggesting that the cysteines of Walker A motifs in both NBFs are responsible for the effects of NEM on ATP binding.	bind
37839	4	8720	5	13	NULL	NULL	NULL	NEM	Chemical		does not inhibit					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1461_2_305_s_156	10581363	8-Azido-ATP binding with the wild-type MDR1 was inhibited by 100  M NEM, while 8-azido-ATP binding with the C431A/C1074A mutant form was not, suggesting that the cysteines of Walker A motifs in both NBFs are responsible for the effects of NEM on ATP binding.	bind
37840	5	8720	5	13	NULL	NULL	NULL	MDR1	GP		contains			NBFs					cysteines in Walker A motifs		NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1461_2_305_s_156	10581363	8-Azido-ATP binding with the wild-type MDR1 was inhibited by 100  M NEM, while 8-azido-ATP binding with the C431A/C1074A mutant form was not, suggesting that the cysteines of Walker A motifs in both NBFs are responsible for the effects of NEM on ATP binding.	bind
37841	6	8720	5	13	NULL	NULL	NULL	statement 5	Process		is responsible for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1461_2_305_s_156	10581363	8-Azido-ATP binding with the wild-type MDR1 was inhibited by 100  M NEM, while 8-azido-ATP binding with the C431A/C1074A mutant form was not, suggesting that the cysteines of Walker A motifs in both NBFs are responsible for the effects of NEM on ATP binding.	bind
36996	1	8720	7	NULL	NULL	0	NULL	8-Azido-ATP	NULL		bind	NULL				MDR1	NULL	wild-type			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1461_2_305_s_156	10581363	8-Azido-ATP binding with the wild-type MDR1 was inhibited by 100  M NEM, while 8-azido-ATP binding with the C431A/C1074A mutant form was not, suggesting that the cysteines of Walker A motifs in both NBFs are responsible for the effects of NEM on ATP binding.	bind
36997	2	8720	7	NULL	NULL	0	NULL	NEM	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1461_2_305_s_156	10581363	8-Azido-ATP binding with the wild-type MDR1 was inhibited by 100  M NEM, while 8-azido-ATP binding with the C431A/C1074A mutant form was not, suggesting that the cysteines of Walker A motifs in both NBFs are responsible for the effects of NEM on ATP binding.	bind
36998	3	8720	7	NULL	NULL	0	NULL	8-Azido-ATP	NULL		bind	NULL				MDR1	NULL	mutant	C431A/C1074A		NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1461_2_305_s_156	10581363	8-Azido-ATP binding with the wild-type MDR1 was inhibited by 100  M NEM, while 8-azido-ATP binding with the C431A/C1074A mutant form was not, suggesting that the cysteines of Walker A motifs in both NBFs are responsible for the effects of NEM on ATP binding.	bind
36999	4	8720	7	NULL	NULL	0	NULL	NEM	NULL		does not inhibit	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1461_2_305_s_156	10581363	8-Azido-ATP binding with the wild-type MDR1 was inhibited by 100  M NEM, while 8-azido-ATP binding with the C431A/C1074A mutant form was not, suggesting that the cysteines of Walker A motifs in both NBFs are responsible for the effects of NEM on ATP binding.	bind
37000	5	8720	7	NULL	NULL	0	NULL	NBF	NULL		is responsible for	NULL		cysteines of Walker A motifs 		statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1461_2_305_s_156	10581363	8-Azido-ATP binding with the wild-type MDR1 was inhibited by 100  M NEM, while 8-azido-ATP binding with the C431A/C1074A mutant form was not, suggesting that the cysteines of Walker A motifs in both NBFs are responsible for the effects of NEM on ATP binding.	bind
37001	6	8720	7	NULL	NULL	0	NULL	NBF	NULL		is responsible for	NULL		cysteines of Walker A motifs 		statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1461_2_305_s_156	10581363	8-Azido-ATP binding with the wild-type MDR1 was inhibited by 100  M NEM, while 8-azido-ATP binding with the C431A/C1074A mutant form was not, suggesting that the cysteines of Walker A motifs in both NBFs are responsible for the effects of NEM on ATP binding.	bind
37842	1	8721	5	13	NULL	NULL	NULL	8-Azido-ATP	Chemical		bind		specifically			TAP1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_32_29686_s_115	12777379	8-Azido-ATP Binds Specifically to TAP1 and TAP2 --	bind
37843	2	8721	5	13	NULL	NULL	NULL	8-Azido-ATP	Chemical		bind		specifically			TAP2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_32_29686_s_115	12777379	8-Azido-ATP Binds Specifically to TAP1 and TAP2 --	bind
37002	1	8721	7	NULL	NULL	0	NULL	8-Azido-ATP	NULL		binds	NULL	specifically			TAP1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_32_29686_s_115	12777379	8-Azido-ATP Binds Specifically to TAP1 and TAP2 --	bind
37003	2	8721	7	NULL	NULL	0	NULL	8-Azido-ATP	NULL		binds	NULL	specifically			TAP2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_32_29686_s_115	12777379	8-Azido-ATP Binds Specifically to TAP1 and TAP2 --	bind
37844	1	8722	5	13	NULL	NULL	NULL	8-Azido-[alpha-32]ATP	Chemical		bind					SURx	GP		NBFs		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_37_28757_s_90	10893240	8-Azido-[alpha-32]ATP binding of NBFs of SURx.	bind
37004	1	8722	7	NULL	NULL	0	NULL	8-Azido-[alpha-32]ATP	NULL		bind	NULL				SURx	NULL		NBFs		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_37_28757_s_90	10893240	8-Azido-[alpha-32]ATP binding of NBFs of SURx.	bind
37845	1	8723	5	13	NULL	NULL	NULL	8-Azido[alpha -32]ATP	Chemical		bind					G5	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_7_4507_s_99	16352607	8-Azido[alpha -32]ATP Binding to G5 and G8 Does Not Require G5G8 Dimerization --	bind
37846	2	8723	5	13	NULL	NULL	NULL	8-Azido[alpha -32]ATP	Chemical		bind					G8	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_7_4507_s_99	16352607	8-Azido[alpha -32]ATP Binding to G5 and G8 Does Not Require G5G8 Dimerization --	bind
37847	3	8723	5	13	NULL	NULL	NULL	statement 1	Process		does not require					G5G8	GP	dimerization of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_7_4507_s_99	16352607	8-Azido[alpha -32]ATP Binding to G5 and G8 Does Not Require G5G8 Dimerization --	bind
37848	4	8723	5	13	NULL	NULL	NULL	statement 2	Process		does not require					G5G8	GP	dimerization of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_7_4507_s_99	16352607	8-Azido[alpha -32]ATP Binding to G5 and G8 Does Not Require G5G8 Dimerization --	bind
37005	1	8723	7	NULL	NULL	0	NULL	8-Azido[alpha -32]ATP	NULL		bind	NULL				G5	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_7_4507_s_99	16352607	8-Azido[alpha -32]ATP Binding to G5 and G8 Does Not Require G5G8 Dimerization --	bind
37006	2	8723	7	NULL	NULL	0	NULL	8-Azido[alpha -32]ATP	NULL		bind	NULL				G8	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_7_4507_s_99	16352607	8-Azido[alpha -32]ATP Binding to G5 and G8 Does Not Require G5G8 Dimerization --	bind
37007	3	8723	7	10	NULL	0	NULL	statement 1			does not require					G5G8 		dimerization of 			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_7_4507_s_99	16352607	8-Azido[alpha -32]ATP Binding to G5 and G8 Does Not Require G5G8 Dimerization --	bind
37008	4	8723	7	10	NULL	0	NULL	statement 2			does not require					G5G8 		dimerization of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_7_4507_s_99	16352607	8-Azido[alpha -32]ATP Binding to G5 and G8 Does Not Require G5G8 Dimerization --	bind
37849	1	8724	5	13	NULL	NULL	NULL	8-Azido[alpha -32]ATP	Chemical		bind					MRP4	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_47_48855_s_92	15364914	8-Azido[alpha -32]ATP Binds to Human MRP4  --	bind
37009	1	8724	7	NULL	NULL	0	NULL	8-Azido[alpha -32]ATP	NULL		binds to	NULL				MRP4	NULL	human			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_47_48855_s_92	15364914	8-Azido[alpha -32]ATP Binds to Human MRP4  --	bind
37850	1	8725	5	13	NULL	NULL	NULL	8-Azido[alpha-32]ATP	Chemical		bind					MRP4	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_47_48855_s_6	15364914	8-Azido[alpha-32]ATP binds to MRP4 (concentration for half-maximal binding  3 muM) and is displaced by ATP or by its non-hydrolyzable analog AMPPNP (concentrations for half-maximal inhibition of 13.3 and 308 muM).	bind
37851	2	8725	5	13	NULL	NULL	NULL	ATP	Chemical		bind					MRP4	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_47_48855_s_6	15364914	8-Azido[alpha-32]ATP binds to MRP4 (concentration for half-maximal binding  3 muM) and is displaced by ATP or by its non-hydrolyzable analog AMPPNP (concentrations for half-maximal inhibition of 13.3 and 308 muM).	bind
37852	3	8725	5	13	NULL	NULL	NULL	statement 2	Process		displaces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_47_48855_s_6	15364914	8-Azido[alpha-32]ATP binds to MRP4 (concentration for half-maximal binding  3 muM) and is displaced by ATP or by its non-hydrolyzable analog AMPPNP (concentrations for half-maximal inhibition of 13.3 and 308 muM).	bind
37853	4	8725	5	13	NULL	NULL	NULL	AMPPNP	Chemical		is an analog of		non-hydrolyzable			8-Azido[alpha-32]ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_47_48855_s_6	15364914	8-Azido[alpha-32]ATP binds to MRP4 (concentration for half-maximal binding  3 muM) and is displaced by ATP or by its non-hydrolyzable analog AMPPNP (concentrations for half-maximal inhibition of 13.3 and 308 muM).	bind
37854	5	8725	5	13	NULL	NULL	NULL	AMPPNP	Chemical		bind					MRP4	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_47_48855_s_6	15364914	8-Azido[alpha-32]ATP binds to MRP4 (concentration for half-maximal binding  3 muM) and is displaced by ATP or by its non-hydrolyzable analog AMPPNP (concentrations for half-maximal inhibition of 13.3 and 308 muM).	bind
37855	6	8725	5	13	NULL	NULL	NULL	statement 5	Process		displaces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_47_48855_s_6	15364914	8-Azido[alpha-32]ATP binds to MRP4 (concentration for half-maximal binding  3 muM) and is displaced by ATP or by its non-hydrolyzable analog AMPPNP (concentrations for half-maximal inhibition of 13.3 and 308 muM).	bind
37856	7	8725	5	13	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_47_48855_s_6	15364914	8-Azido[alpha-32]ATP binds to MRP4 (concentration for half-maximal binding  3 muM) and is displaced by ATP or by its non-hydrolyzable analog AMPPNP (concentrations for half-maximal inhibition of 13.3 and 308 muM).	bind
37010	1	8725	7	NULL	NULL	0	NULL	8-Azido[alpha-32]ATP	NULL		binds to	NULL				MRP4	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_47_48855_s_6	15364914	8-Azido[alpha-32]ATP binds to MRP4 (concentration for half-maximal binding  3 muM) and is displaced by ATP or by its non-hydrolyzable analog AMPPNP (concentrations for half-maximal inhibition of 13.3 and 308 muM).	bind
37011	2	8725	7	NULL	NULL	0	NULL	ATP	NULL		bind	NULL				MRP4	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_47_48855_s_6	15364914	8-Azido[alpha-32]ATP binds to MRP4 (concentration for half-maximal binding  3 muM) and is displaced by ATP or by its non-hydrolyzable analog AMPPNP (concentrations for half-maximal inhibition of 13.3 and 308 muM).	bind
37012	3	8725	7	NULL	NULL	0	NULL	statement 2	NULL		displace	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_47_48855_s_6	15364914	8-Azido[alpha-32]ATP binds to MRP4 (concentration for half-maximal binding  3 muM) and is displaced by ATP or by its non-hydrolyzable analog AMPPNP (concentrations for half-maximal inhibition of 13.3 and 308 muM).	bind
37013	4	8725	7	NULL	NULL	0	NULL	AMPPNP	NULL		bind	NULL				MRP4	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_47_48855_s_6	15364914	8-Azido[alpha-32]ATP binds to MRP4 (concentration for half-maximal binding  3 muM) and is displaced by ATP or by its non-hydrolyzable analog AMPPNP (concentrations for half-maximal inhibition of 13.3 and 308 muM).	bind
37014	5	8725	7	NULL	NULL	0	NULL	statement 4	NULL		displace	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_47_48855_s_6	15364914	8-Azido[alpha-32]ATP binds to MRP4 (concentration for half-maximal binding  3 muM) and is displaced by ATP or by its non-hydrolyzable analog AMPPNP (concentrations for half-maximal inhibition of 13.3 and 308 muM).	bind
37015	6	8725	7	NULL	NULL	0	NULL	AMPPNP	NULL		is a type of	NULL				non-hydrolyzable analog	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_47_48855_s_6	15364914	8-Azido[alpha-32]ATP binds to MRP4 (concentration for half-maximal binding  3 muM) and is displaced by ATP or by its non-hydrolyzable analog AMPPNP (concentrations for half-maximal inhibition of 13.3 and 308 muM).	bind
38741	1	8726	5	13	NULL	NULL	NULL	8-Cl-cAMP	Chemical		targets		specifically			PKA	GP		cAMP binding sites in regulatory R-I subunit		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_34_21137_s_78	9261118	8-Cl-cAMP specifically targets the high affinity cAMP binding sites in the regulatory R-I subunit of PKA ( 35), which results in the sustained activation and proteolysis of type I PKA and the down-regulation of cAMP-dependent transcription factors ( 26,  28).	bind
38742	2	8726	5	13	NULL	NULL	NULL	statement 1	Process		results in					type I PKA	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_34_21137_s_78	9261118	8-Cl-cAMP specifically targets the high affinity cAMP binding sites in the regulatory R-I subunit of PKA ( 35), which results in the sustained activation and proteolysis of type I PKA and the down-regulation of cAMP-dependent transcription factors ( 26,  28).	bind
38743	3	8726	5	13	NULL	NULL	NULL	statement 1	Process		results in					type I PKA	GP	proteolysis of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_34_21137_s_78	9261118	8-Cl-cAMP specifically targets the high affinity cAMP binding sites in the regulatory R-I subunit of PKA ( 35), which results in the sustained activation and proteolysis of type I PKA and the down-regulation of cAMP-dependent transcription factors ( 26,  28).	bind
38744	4	8726	5	13	NULL	NULL	NULL	statement 1	Process		results in					cAMP-dependent transcription factors	GP	down-regulation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_34_21137_s_78	9261118	8-Cl-cAMP specifically targets the high affinity cAMP binding sites in the regulatory R-I subunit of PKA ( 35), which results in the sustained activation and proteolysis of type I PKA and the down-regulation of cAMP-dependent transcription factors ( 26,  28).	bind
37083	1	8726	7	NULL	NULL	0	NULL	8-Cl-cAMP	NULL		targets	NULL	specifically			pKA	NULL		cAMP binding sites in the regulatory R-I subunit		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_34_21137_s_78	9261118	8-Cl-cAMP specifically targets the high affinity cAMP binding sites in the regulatory R-I subunit of PKA ( 35), which results in the sustained activation and proteolysis of type I PKA and the down-regulation of cAMP-dependent transcription factors ( 26,  28).	bind
37084	2	8726	7	NULL	NULL	0	NULL	statement 1	NULL		results in	NULL				type I PKA	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_34_21137_s_78	9261118	8-Cl-cAMP specifically targets the high affinity cAMP binding sites in the regulatory R-I subunit of PKA ( 35), which results in the sustained activation and proteolysis of type I PKA and the down-regulation of cAMP-dependent transcription factors ( 26,  28).	bind
37085	3	8726	7	NULL	NULL	0	NULL	statement 1	NULL		results in	NULL				type I PKA	NULL	proteolysis of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_34_21137_s_78	9261118	8-Cl-cAMP specifically targets the high affinity cAMP binding sites in the regulatory R-I subunit of PKA ( 35), which results in the sustained activation and proteolysis of type I PKA and the down-regulation of cAMP-dependent transcription factors ( 26,  28).	bind
37086	4	8726	7	NULL	NULL	0	NULL	statement 1	NULL		results in	NULL				cAMP-dependent transcription factors 	NULL	down-regulation of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_34_21137_s_78	9261118	8-Cl-cAMP specifically targets the high affinity cAMP binding sites in the regulatory R-I subunit of PKA ( 35), which results in the sustained activation and proteolysis of type I PKA and the down-regulation of cAMP-dependent transcription factors ( 26,  28).	bind
37947	1	8727	5	13	NULL	NULL	NULL	8-N3-[32]cAMP	Chemical		bind					52 kDa protein	GP				NULL	microtubule fraction from total cortex of rats treated with vehicle	NULL	NULL	NULL	NULL	gw60_neuropharmacology_40_3_448_s_97	11166338	8-N3-[32]cAMP binding to the 52 kDa protein band (indicated by arrow) in microtubule fraction from total cortex of rats treated with vehicle (1, 2) or reboxetine (3, 4).	bind
37948	2	8727	5	13	NULL	NULL	NULL	8-N3-[32]cAMP	Chemical		bind					52 kDa protein	GP				NULL	microtubule fraction from total cortex of rats treated with reboxetine	NULL	NULL	NULL	NULL	gw60_neuropharmacology_40_3_448_s_97	11166338	8-N3-[32]cAMP binding to the 52 kDa protein band (indicated by arrow) in microtubule fraction from total cortex of rats treated with vehicle (1, 2) or reboxetine (3, 4).	bind
37956	3	8727	5	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_40_3_448_s_97	11166338	8-N3-[32]cAMP binding to the 52 kDa protein band (indicated by arrow) in microtubule fraction from total cortex of rats treated with vehicle (1, 2) or reboxetine (3, 4).	bind
37087	1	8727	7	NULL	NULL	0	NULL	8-N3-[32]cAMP	NULL		bind	NULL				52 kDa protein 	NULL				NULL	vehicle treated microtubule fraction from total cortex of rats	0	NULL	NULL	NULL	gw60_neuropharmacology_40_3_448_s_97	11166338	8-N3-[32]cAMP binding to the 52 kDa protein band (indicated by arrow) in microtubule fraction from total cortex of rats treated with vehicle (1, 2) or reboxetine (3, 4).	bind
37088	2	8727	7	NULL	NULL	0	NULL	8-N3-[32]cAMP	NULL		bind	NULL				52 kDa protein 	NULL				NULL	reboxetine treated microtubule fraction from total cortex of rats	0	NULL	NULL	NULL	gw60_neuropharmacology_40_3_448_s_97	11166338	8-N3-[32]cAMP binding to the 52 kDa protein band (indicated by arrow) in microtubule fraction from total cortex of rats treated with vehicle (1, 2) or reboxetine (3, 4).	bind
46754	3	8727	7	10	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_40_3_448_s_97	11166338	8-N3-[32]cAMP binding to the 52 kDa protein band (indicated by arrow) in microtubule fraction from total cortex of rats treated with vehicle (1, 2) or reboxetine (3, 4).	bind
37957	1	8728	5	13	NULL	NULL	NULL	8-N3-[32]cAMP	Chemical		bind					52 kDa protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_40_3_448_s_104	11166338	8-N3-[32]cAMP binding to the 52 kDa protein band (indicated by arrows) in	bind
37089	1	8728	7	NULL	NULL	0	NULL	8-N3-[32]cAMP	NULL		bind	NULL				52 kDa protein 	NULL				NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_40_3_448_s_104	11166338	8-N3-[32]cAMP binding to the 52 kDa protein band (indicated by arrows) in	bind
37959	1	8729	5	13	NULL	NULL	NULL	FdUMP	Chemical		bind					enzyme	GP	wild-type			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_31_28901_s_260	12754260	80% of *FdUMP remains bound  to the  wild-type enzyme in the presence of excess CH2H4folate  and dUMP, whereas only 33% remains bound to the K282E/R283E mutant.	bind
37961	2	8729	5	13	NULL	NULL	NULL	statement 1	Process		in the presence of					CH2H4folate	Chemical	excess			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_31_28901_s_260	12754260	80% of *FdUMP remains bound  to the  wild-type enzyme in the presence of excess CH2H4folate  and dUMP, whereas only 33% remains bound to the K282E/R283E mutant.	bind
37962	3	8729	5	13	NULL	NULL	NULL	statement 1	Process		in the presence of					dUMP	Chemical	excess			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_31_28901_s_260	12754260	80% of *FdUMP remains bound  to the  wild-type enzyme in the presence of excess CH2H4folate  and dUMP, whereas only 33% remains bound to the K282E/R283E mutant.	bind
37963	4	8729	5	13	NULL	NULL	NULL	FdUMP	Chemical		bind					enzyme	GP	mutant	K282E/R283E		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_31_28901_s_260	12754260	80% of *FdUMP remains bound  to the  wild-type enzyme in the presence of excess CH2H4folate  and dUMP, whereas only 33% remains bound to the K282E/R283E mutant.	bind
37090	1	8729	7	NULL	NULL	0	NULL	FdUMP 	NULL		bind	NULL				enzyme	NULL	wild-type			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_31_28901_s_260	12754260	80% of *FdUMP remains bound  to the  wild-type enzyme in the presence of excess CH2H4folate  and dUMP, whereas only 33% remains bound to the K282E/R283E mutant.	bind
37091	2	8729	7	10	NULL	0	NULL	statement 1			in presence of					CH2H4folate		excess			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_31_28901_s_260	12754260	80% of *FdUMP remains bound  to the  wild-type enzyme in the presence of excess CH2H4folate  and dUMP, whereas only 33% remains bound to the K282E/R283E mutant.	bind
37092	3	8729	7	10	NULL	0	NULL	statement 1			in presence of					dUMP		excess			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_31_28901_s_260	12754260	80% of *FdUMP remains bound  to the  wild-type enzyme in the presence of excess CH2H4folate  and dUMP, whereas only 33% remains bound to the K282E/R283E mutant.	bind
37093	4	8729	7	NULL	NULL	0	NULL	FdUMP 	NULL		bind	NULL				enzyme	NULL	mutant	K282E/R283E		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_31_28901_s_260	12754260	80% of *FdUMP remains bound  to the  wild-type enzyme in the presence of excess CH2H4folate  and dUMP, whereas only 33% remains bound to the K282E/R283E mutant.	bind
37964	1	8730	5	13	NULL	NULL	NULL	80K-H protein	GP		bind		specifically			TRPV5	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_25_26351_s_99	15100231	80K-H protein bound specifically to TRPV5 in both conditions because no interaction was observed with GST alone ( Fig. 2 C).	bind
37094	1	8730	7	NULL	NULL	0	NULL	80K-H protein	NULL		bind	NULL	specifically			TRPV5	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_25_26351_s_99	15100231	80K-H protein bound specifically to TRPV5 in both conditions because no interaction was observed with GST alone ( Fig. 2 C).	bind
37857	1	8731	5	13	NULL	NULL	NULL	S1	GP		bind					ACE2 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_8_2536_s_136	14983044	80R scFv inhibiting the binding of S1 to ACE2 receptor.	bind
37858	2	8731	5	13	NULL	NULL	NULL	80R scFv	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_8_2536_s_136	14983044	80R scFv inhibiting the binding of S1 to ACE2 receptor.	bind
37095	1	8731	7	NULL	NULL	0	NULL	S1	NULL		bind	NULL				ACE2 receptor	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_101_8_2536_s_136	14983044	80R scFv inhibiting the binding of S1 to ACE2 receptor.	bind
37096	2	8731	7	NULL	NULL	0	NULL	80R scFv	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_101_8_2536_s_136	14983044	80R scFv inhibiting the binding of S1 to ACE2 receptor.	bind
37859	1	8732	5	13	NULL	NULL	NULL	Rac1	GP		bind					p67 phox	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_4_453_s_162	16514078	86 This region is not required for Rac1 binding to p67 phox, implicating another protein, binding to this domain, in the activation of the oxidase.	bind
37097	1	8732	7	NULL	NULL	0	NULL	Rac1	NULL		bind	NULL				p67 phox	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_4_453_s_162	16514078	86 This region is not required for Rac1 binding to p67 phox, implicating another protein, binding to this domain, in the activation of the oxidase.	bind
37860	1	8733	5	13	NULL	NULL	NULL	synectin	GP		bind					syndecan-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_5_488_s_172	15774861	87 However, synectin also binds syndecan-2.	bind
37098	1	8733	7	NULL	NULL	0	NULL	synectin	NULL		bind	NULL				 syndecan-2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_5_488_s_172	15774861	87 However, synectin also binds syndecan-2.	bind
37861	1	8734	5	13	NULL	NULL	NULL	ezrin	GP		links					syndecan-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_824_s_141	14976004	87,88  Moreover, it appears that ezrin links the proteoglycan syndecan-2, which might possibly bind SDF-1, to the actin cytoskeleton.	bind
37862	2	8734	5	13	NULL	NULL	NULL	syndecan-2	GP		is a type of					proteoglycan	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_824_s_141	14976004	87,88  Moreover, it appears that ezrin links the proteoglycan syndecan-2, which might possibly bind SDF-1, to the actin cytoskeleton.	bind
37863	3	8734	5	13	NULL	NULL	NULL	SDF-1	GP		bind					actin cytoskeleton	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_824_s_141	14976004	87,88  Moreover, it appears that ezrin links the proteoglycan syndecan-2, which might possibly bind SDF-1, to the actin cytoskeleton.	bind
37864	4	8734	5	13	NULL	NULL	NULL	syndecan-2	GP		is required for		possibly			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_824_s_141	14976004	87,88  Moreover, it appears that ezrin links the proteoglycan syndecan-2, which might possibly bind SDF-1, to the actin cytoskeleton.	bind
37099	1	8734	7	NULL	NULL	0	NULL	ezrin	NULL		links	NULL				syndecan-2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_824_s_141	14976004	87,88  Moreover, it appears that ezrin links the proteoglycan syndecan-2, which might possibly bind SDF-1, to the actin cytoskeleton.	bind
37100	2	8734	7	NULL	NULL	0	NULL	SDF-1	NULL		bind	NULL				actin cytoskeleton	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_824_s_141	14976004	87,88  Moreover, it appears that ezrin links the proteoglycan syndecan-2, which might possibly bind SDF-1, to the actin cytoskeleton.	bind
37101	3	8734	7	NULL	NULL	0	NULL	syndecan-2	NULL		is a type of	NULL				proteoglycan	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_824_s_141	14976004	87,88  Moreover, it appears that ezrin links the proteoglycan syndecan-2, which might possibly bind SDF-1, to the actin cytoskeleton.	bind
46756	4	8734	7	10	NULL	0	NULL	syndecan-2	NULL		is involved in	NULL	possibly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_824_s_141	14976004	87,88  Moreover, it appears that ezrin links the proteoglycan syndecan-2, which might possibly bind SDF-1, to the actin cytoskeleton.	bind
37865	1	8735	5	13	NULL	NULL	NULL	Mcl-1	GP		bind					Bak	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_118	15539639	88 On initiation of apoptosis, VDAC2 is displaced from Bak by activated (truncated) Bid, Bim, and Bad, whereas Mcl-1 binding to Bak is disrupted by p53.	bind
37866	2	8735	5	13	NULL	NULL	NULL	p53	GP		disrupt					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_118	15539639	88 On initiation of apoptosis, VDAC2 is displaced from Bak by activated (truncated) Bid, Bim, and Bad, whereas Mcl-1 binding to Bak is disrupted by p53.	bind
37867	3	8735	5	13	NULL	NULL	NULL	statement 2	Process		occurs during					apoptosis	Process	initiation of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_118	15539639	88 On initiation of apoptosis, VDAC2 is displaced from Bak by activated (truncated) Bid, Bim, and Bad, whereas Mcl-1 binding to Bak is disrupted by p53.	bind
37868	4	8735	5	13	NULL	NULL	NULL	VDAC2	GP		bind					Bak	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_118	15539639	88 On initiation of apoptosis, VDAC2 is displaced from Bak by activated (truncated) Bid, Bim, and Bad, whereas Mcl-1 binding to Bak is disrupted by p53.	bind
37869	5	8735	5	13	NULL	NULL	NULL	Bid	GP	activated;;truncated	bind					Bak	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_118	15539639	88 On initiation of apoptosis, VDAC2 is displaced from Bak by activated (truncated) Bid, Bim, and Bad, whereas Mcl-1 binding to Bak is disrupted by p53.	bind
37870	6	8735	5	13	NULL	NULL	NULL	statement 5	Process		displaces					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_118	15539639	88 On initiation of apoptosis, VDAC2 is displaced from Bak by activated (truncated) Bid, Bim, and Bad, whereas Mcl-1 binding to Bak is disrupted by p53.	bind
37871	7	8735	5	13	NULL	NULL	NULL	statement 6	Process		occurs during					apoptosis	Process	initiation of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_118	15539639	88 On initiation of apoptosis, VDAC2 is displaced from Bak by activated (truncated) Bid, Bim, and Bad, whereas Mcl-1 binding to Bak is disrupted by p53.	bind
38756	8	8735	5	13	NULL	NULL	NULL	Bim	GP	activated;;truncated	bind					Bak	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_118	15539639	88 On initiation of apoptosis, VDAC2 is displaced from Bak by activated (truncated) Bid, Bim, and Bad, whereas Mcl-1 binding to Bak is disrupted by p53.	bind
38757	9	8735	5	13	NULL	NULL	NULL	statement 8	Process		displaces					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_118	15539639	88 On initiation of apoptosis, VDAC2 is displaced from Bak by activated (truncated) Bid, Bim, and Bad, whereas Mcl-1 binding to Bak is disrupted by p53.	bind
38758	10	8735	5	13	NULL	NULL	NULL	statement 9	Process		occurs during					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_118	15539639	88 On initiation of apoptosis, VDAC2 is displaced from Bak by activated (truncated) Bid, Bim, and Bad, whereas Mcl-1 binding to Bak is disrupted by p53.	bind
38759	11	8735	5	13	NULL	NULL	NULL	Bad	GP	activated;;truncated	bind					Bak	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_118	15539639	88 On initiation of apoptosis, VDAC2 is displaced from Bak by activated (truncated) Bid, Bim, and Bad, whereas Mcl-1 binding to Bak is disrupted by p53.	bind
38760	12	8735	5	13	NULL	NULL	NULL	statement 11	Process		displaces					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_118	15539639	88 On initiation of apoptosis, VDAC2 is displaced from Bak by activated (truncated) Bid, Bim, and Bad, whereas Mcl-1 binding to Bak is disrupted by p53.	bind
38762	13	8735	5	13	NULL	NULL	NULL	statement 12	Process		occurs during					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_118	15539639	88 On initiation of apoptosis, VDAC2 is displaced from Bak by activated (truncated) Bid, Bim, and Bad, whereas Mcl-1 binding to Bak is disrupted by p53.	bind
37102	4	8735	7	10	NULL	0	NULL	VDAC2			bind					Bak					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_118	15539639	88 On initiation of apoptosis, VDAC2 is displaced from Bak by activated (truncated) Bid, Bim, and Bad, whereas Mcl-1 binding to Bak is disrupted by p53.	bind
37103	3	8735	7	10	NULL	0	NULL	statement 2			occurs upon					apoptosis		initiation of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_118	15539639	88 On initiation of apoptosis, VDAC2 is displaced from Bak by activated (truncated) Bid, Bim, and Bad, whereas Mcl-1 binding to Bak is disrupted by p53.	bind
37104	5	8735	7	10	NULL	0	NULL	Bid		acitvated;;truncated	bind					Bak					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_118	15539639	88 On initiation of apoptosis, VDAC2 is displaced from Bak by activated (truncated) Bid, Bim, and Bad, whereas Mcl-1 binding to Bak is disrupted by p53.	bind
37105	6	8735	7	10	NULL	0	NULL	statement 5			displaces					statement 4					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_118	15539639	88 On initiation of apoptosis, VDAC2 is displaced from Bak by activated (truncated) Bid, Bim, and Bad, whereas Mcl-1 binding to Bak is disrupted by p53.	bind
37106	7	8735	7	10	NULL	0	NULL	statement 6			occurs during					apoptosis		initiation of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_118	15539639	88 On initiation of apoptosis, VDAC2 is displaced from Bak by activated (truncated) Bid, Bim, and Bad, whereas Mcl-1 binding to Bak is disrupted by p53.	bind
37107	1	8735	7	10	NULL	0	NULL	Mcl-1			bind					Bak					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_118	15539639	88 On initiation of apoptosis, VDAC2 is displaced from Bak by activated (truncated) Bid, Bim, and Bad, whereas Mcl-1 binding to Bak is disrupted by p53.	bind
37108	2	8735	7	10	NULL	0	NULL	p53			disrupts					statement 1					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_118	15539639	88 On initiation of apoptosis, VDAC2 is displaced from Bak by activated (truncated) Bid, Bim, and Bad, whereas Mcl-1 binding to Bak is disrupted by p53.	bind
56479	8	8735	7	10	NULL	0	NULL	Bim		activated;;truncated	bind					Bak					NULL		0	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_118	15539639	88 On initiation of apoptosis, VDAC2 is displaced from Bak by activated (truncated) Bid, Bim, and Bad, whereas Mcl-1 binding to Bak is disrupted by p53.	bind
56480	9	8735	7	10	NULL	0	NULL	statement 8			displaces					statement 4					NULL		0	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_118	15539639	88 On initiation of apoptosis, VDAC2 is displaced from Bak by activated (truncated) Bid, Bim, and Bad, whereas Mcl-1 binding to Bak is disrupted by p53.	bind
56481	10	8735	7	10	NULL	0	NULL	statement 9			occur during					apoptosis		initiation of			NULL		0	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_118	15539639	88 On initiation of apoptosis, VDAC2 is displaced from Bak by activated (truncated) Bid, Bim, and Bad, whereas Mcl-1 binding to Bak is disrupted by p53.	bind
56482	11	8735	7	10	NULL	0	NULL	Bad		activated;;truncated	bind					Bak					NULL		0	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_118	15539639	88 On initiation of apoptosis, VDAC2 is displaced from Bak by activated (truncated) Bid, Bim, and Bad, whereas Mcl-1 binding to Bak is disrupted by p53.	bind
56483	12	8735	7	10	NULL	0	NULL	statement 11			displaces					statement 4					NULL		0	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_118	15539639	88 On initiation of apoptosis, VDAC2 is displaced from Bak by activated (truncated) Bid, Bim, and Bad, whereas Mcl-1 binding to Bak is disrupted by p53.	bind
56484	13	8735	7	10	NULL	0	NULL	statement 12			occur during					apoptosis		initiation of			NULL		0	NULL	NULL	NULL	gw70_circulationres_95_10_957_s_118	15539639	88 On initiation of apoptosis, VDAC2 is displaced from Bak by activated (truncated) Bid, Bim, and Bad, whereas Mcl-1 binding to Bak is disrupted by p53.	bind
37872	1	8736	5	13	NULL	NULL	NULL	amphotericin B	Chemical		is a type of					antibiotic	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_11_1182_s_209	12805236	88,89  Treatment with amphotericin B, an antibiotic that binds cholesterol, causes the disruption of t-tubules in C2C12 myotubes.	bind
37873	2	8736	5	13	NULL	NULL	NULL	amphotericin B	Chemical		bind					cholesterol	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_11_1182_s_209	12805236	88,89  Treatment with amphotericin B, an antibiotic that binds cholesterol, causes the disruption of t-tubules in C2C12 myotubes.	bind
37874	3	8736	5	13	NULL	NULL	NULL	statement 2	Process		disrupt					t-tubules	OrganismPart				NULL	C2C12 myotubes	NULL	NULL	NULL	NULL	gw70_circulationres_92_11_1182_s_209	12805236	88,89  Treatment with amphotericin B, an antibiotic that binds cholesterol, causes the disruption of t-tubules in C2C12 myotubes.	bind
37109	1	8736	7	NULL	NULL	0	NULL	amphotericin B	NULL		binds	NULL				cholesterol	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_92_11_1182_s_209	12805236	88,89  Treatment with amphotericin B, an antibiotic that binds cholesterol, causes the disruption of t-tubules in C2C12 myotubes.	bind
37110	2	8736	7	NULL	NULL	0	NULL	amphotericin B	NULL		is a type of	NULL				antibiotic	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_92_11_1182_s_209	12805236	88,89  Treatment with amphotericin B, an antibiotic that binds cholesterol, causes the disruption of t-tubules in C2C12 myotubes.	bind
37111	3	8736	7	10	NULL	0	NULL	statement 1	NULL		disrupts	NULL				t-tubules	NULL				NULL	C2C12 myotubes	NULL	NULL	NULL	NULL	gw70_circulationres_92_11_1182_s_209	12805236	88,89  Treatment with amphotericin B, an antibiotic that binds cholesterol, causes the disruption of t-tubules in C2C12 myotubes.	bind
37892	1	8737	5	13	NULL	NULL	NULL	EGF	GP		stimulate					MAPK	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_3_1671_s_120	11805301	8Br-cAMP did not inhibit EGF stimulation of MAPK (Fig.  2 A).	bind
37893	2	8737	5	13	NULL	NULL	NULL	8Br-cAMP	Chemical		does not inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_3_1671_s_120	11805301	8Br-cAMP did not inhibit EGF stimulation of MAPK (Fig.  2 A).	bind
37138	1	8737	7	NULL	NULL	0	NULL	EGF	NULL		stimulates	NULL				MAPK	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_3_1671_s_120	11805301	8Br-cAMP did not inhibit EGF stimulation of MAPK (Fig.  2 A).	bind
37139	2	8737	7	NULL	NULL	0	NULL	8Br-cAMP	NULL		does not inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_3_1671_s_120	11805301	8Br-cAMP did not inhibit EGF stimulation of MAPK (Fig.  2 A).	bind
37894	1	8738	5	13	NULL	NULL	NULL	Pax6	GP		controls					radial glia	OrganismPart	differentiation of			NULL	cerebral cortex	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_19_4070_s_251	11574690	9       Gotz,M., Stoykova,A. and Gruss,P. (1998) Pax6 controls radial glia differentiation in the cerebral cortex.	bind
37140	1	8738	7	10	NULL	0	NULL	Pax6 	NULL		controls	NULL				 radial glia 	NULL	differentiation 			NULL	cerebral cortex	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_19_4070_s_251	11574690	9       Gotz,M., Stoykova,A. and Gruss,P. (1998) Pax6 controls radial glia differentiation in the cerebral cortex.	bind
37895	1	8740	5	13	NULL	NULL	NULL	VP16	GP		bind			acidic transcriptional activation domains		replication protein A	GP	cellular			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_15_3270_s_216	11470885	9       Li,R. and Botchan,M.R. (1993) The acidic transcriptional activation domains of VP16 and p53 bind the cellular replication protein A and stimulate  in vitro BPV-1 DNA replication.	bind
37896	2	8740	5	13	NULL	NULL	NULL	statement 1	Process		stimulate					BPV-1 DNA	NucleicAcid	replication of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_15_3270_s_216	11470885	9       Li,R. and Botchan,M.R. (1993) The acidic transcriptional activation domains of VP16 and p53 bind the cellular replication protein A and stimulate  in vitro BPV-1 DNA replication.	bind
37897	3	8740	5	13	NULL	NULL	NULL	p53	GP		bind			acidic transcriptional activation domains		replication protein A	GP	cellular			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_15_3270_s_216	11470885	9       Li,R. and Botchan,M.R. (1993) The acidic transcriptional activation domains of VP16 and p53 bind the cellular replication protein A and stimulate  in vitro BPV-1 DNA replication.	bind
37898	4	8740	5	13	NULL	NULL	NULL	statement 3	Process		stimulate					BPV-1 DNA	NucleicAcid	replication of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_15_3270_s_216	11470885	9       Li,R. and Botchan,M.R. (1993) The acidic transcriptional activation domains of VP16 and p53 bind the cellular replication protein A and stimulate  in vitro BPV-1 DNA replication.	bind
37141	1	8740	7	NULL	NULL	0	NULL	VP16	NULL		bind	NULL		acidic transcriptional activation domains of		cellular replication protein A	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_15_3270_s_216	11470885	9       Li,R. and Botchan,M.R. (1993) The acidic transcriptional activation domains of VP16 and p53 bind the cellular replication protein A and stimulate  in vitro BPV-1 DNA replication.	bind
37142	2	8740	7	10	NULL	0	NULL	p53	NULL		bind	NULL		acidic transcriptional activation domain		cellular replication protein A	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_15_3270_s_216	11470885	9       Li,R. and Botchan,M.R. (1993) The acidic transcriptional activation domains of VP16 and p53 bind the cellular replication protein A and stimulate  in vitro BPV-1 DNA replication.	bind
37143	3	8740	7	NULL	NULL	0	NULL	statement 1	NULL		stimulate	NULL				BPV-1 DNA	NULL	replication of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_15_3270_s_216	11470885	9       Li,R. and Botchan,M.R. (1993) The acidic transcriptional activation domains of VP16 and p53 bind the cellular replication protein A and stimulate  in vitro BPV-1 DNA replication.	bind
37144	4	8740	7	NULL	NULL	0	NULL	statement 2	NULL		stimulate	NULL				BPV-1 DNA	NULL	replication of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_15_3270_s_216	11470885	9       Li,R. and Botchan,M.R. (1993) The acidic transcriptional activation domains of VP16 and p53 bind the cellular replication protein A and stimulate  in vitro BPV-1 DNA replication.	bind
37899	1	8741	5	13	NULL	NULL	NULL	CRP	GP		bind					LDL	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2094_s_181	10978254	9  10 11  (2) CRP displays in vitro binding to LDL and, thus, may be entrapped in the intima by deposited lipids.	bind
37900	2	8741	5	13	NULL	NULL	NULL	lipids	Chemical	deposited	entrap					statement 1	Process				NULL	intima	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2094_s_181	10978254	9  10 11  (2) CRP displays in vitro binding to LDL and, thus, may be entrapped in the intima by deposited lipids.	bind
37145	1	8741	7	NULL	NULL	0	NULL	CRP 	NULL		bind	NULL				LDL	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2094_s_181	10978254	9  10 11  (2) CRP displays in vitro binding to LDL and, thus, may be entrapped in the intima by deposited lipids.	bind
37146	2	8741	7	NULL	NULL	0	NULL	CRP	NULL		is entrapped in	NULL				intima 	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2094_s_181	10978254	9  10 11  (2) CRP displays in vitro binding to LDL and, thus, may be entrapped in the intima by deposited lipids.	bind
37147	3	8741	7	NULL	NULL	0	NULL	statement 2	NULL		occurs by	NULL				deposited lipids	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2094_s_181	10978254	9  10 11  (2) CRP displays in vitro binding to LDL and, thus, may be entrapped in the intima by deposited lipids.	bind
38734	1	8742	5	13	NULL	NULL	NULL	selectins	GP		bind		high affinity			SLex	Chemical	sialylated;;fucosylated			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_1_93_s_361	null	9  14  All 3 selectins demonstrate a high affinity for sialylated, fucosylated saccharide structures such as SLex, and although there are several leukocyte-bound structures that present SLex, it appears as though P-selectin must bind with PSGL-1 in order for leukocytes to efficiently roll along the endothelium under physiological flow conditions.	bind
38735	2	8742	5	13	NULL	NULL	NULL	SLex	Chemical		is a type of					saccharide	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_1_93_s_361	null	9  14  All 3 selectins demonstrate a high affinity for sialylated, fucosylated saccharide structures such as SLex, and although there are several leukocyte-bound structures that present SLex, it appears as though P-selectin must bind with PSGL-1 in order for leukocytes to efficiently roll along the endothelium under physiological flow conditions.	bind
38736	3	8742	5	13	NULL	NULL	NULL	leukocyte-bound structures	Chemical		present					SLex	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_1_93_s_361	null	9  14  All 3 selectins demonstrate a high affinity for sialylated, fucosylated saccharide structures such as SLex, and although there are several leukocyte-bound structures that present SLex, it appears as though P-selectin must bind with PSGL-1 in order for leukocytes to efficiently roll along the endothelium under physiological flow conditions.	bind
38737	4	8742	5	13	NULL	NULL	NULL	P-selectin	GP		bind		possibly			PSGL-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_1_93_s_361	null	9  14  All 3 selectins demonstrate a high affinity for sialylated, fucosylated saccharide structures such as SLex, and although there are several leukocyte-bound structures that present SLex, it appears as though P-selectin must bind with PSGL-1 in order for leukocytes to efficiently roll along the endothelium under physiological flow conditions.	bind
38738	5	8742	5	13	NULL	NULL	NULL	leukocytes	Cell		roll along		efficiently			endothelium	Cell				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_1_93_s_361	null	9  14  All 3 selectins demonstrate a high affinity for sialylated, fucosylated saccharide structures such as SLex, and although there are several leukocyte-bound structures that present SLex, it appears as though P-selectin must bind with PSGL-1 in order for leukocytes to efficiently roll along the endothelium under physiological flow conditions.	bind
38740	7	8742	5	13	NULL	NULL	NULL	statement 5	Process		requires					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_1_93_s_361	null	9  14  All 3 selectins demonstrate a high affinity for sialylated, fucosylated saccharide structures such as SLex, and although there are several leukocyte-bound structures that present SLex, it appears as though P-selectin must bind with PSGL-1 in order for leukocytes to efficiently roll along the endothelium under physiological flow conditions.	bind
56357	6	8742	5	13	NULL	NULL	NULL	statement 2	Process		occurs under					physiological flow conditions					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_1_93_s_361	null	9  14  All 3 selectins demonstrate a high affinity for sialylated, fucosylated saccharide structures such as SLex, and although there are several leukocyte-bound structures that present SLex, it appears as though P-selectin must bind with PSGL-1 in order for leukocytes to efficiently roll along the endothelium under physiological flow conditions.	bind
37148	1	8742	7	NULL	NULL	0	NULL	P-selectin 	NULL		bind	NULL				PSGL-1 	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_1_93_s_361	null	9  14  All 3 selectins demonstrate a high affinity for sialylated, fucosylated saccharide structures such as SLex, and although there are several leukocyte-bound structures that present SLex, it appears as though P-selectin must bind with PSGL-1 in order for leukocytes to efficiently roll along the endothelium under physiological flow conditions.	bind
37149	2	8742	7	10	NULL	0	NULL	leukocytes			roll along		efficiently			endothelium					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_1_93_s_361	null	9  14  All 3 selectins demonstrate a high affinity for sialylated, fucosylated saccharide structures such as SLex, and although there are several leukocyte-bound structures that present SLex, it appears as though P-selectin must bind with PSGL-1 in order for leukocytes to efficiently roll along the endothelium under physiological flow conditions.	bind
37150	4	8742	7	NULL	NULL	0	NULL	 selectins 	NULL		demonstrate	NULL	high affinity			SLex	NULL	sialylated			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_1_93_s_361	null	9  14  All 3 selectins demonstrate a high affinity for sialylated, fucosylated saccharide structures such as SLex, and although there are several leukocyte-bound structures that present SLex, it appears as though P-selectin must bind with PSGL-1 in order for leukocytes to efficiently roll along the endothelium under physiological flow conditions.	bind
37151	3	8742	7	NULL	NULL	0	NULL	statement 1	NULL		is required for	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_1_93_s_361	null	9  14  All 3 selectins demonstrate a high affinity for sialylated, fucosylated saccharide structures such as SLex, and although there are several leukocyte-bound structures that present SLex, it appears as though P-selectin must bind with PSGL-1 in order for leukocytes to efficiently roll along the endothelium under physiological flow conditions.	bind
37152	5	8742	7	NULL	NULL	0	NULL	selectins	NULL		demonstrate	NULL	high affinity			SLex	NULL	fucosylated			NULL		0	NULL	NULL	NULL	gw60_circulationres_84_1_93_s_361	null	9  14  All 3 selectins demonstrate a high affinity for sialylated, fucosylated saccharide structures such as SLex, and although there are several leukocyte-bound structures that present SLex, it appears as though P-selectin must bind with PSGL-1 in order for leukocytes to efficiently roll along the endothelium under physiological flow conditions.	bind
56358	6	8742	7	10	NULL	0	NULL	statement 2			occurs under					physiological flow conditions					NULL		0	NULL	NULL	NULL	gw60_circulationres_84_1_93_s_361	null	9  14  All 3 selectins demonstrate a high affinity for sialylated, fucosylated saccharide structures such as SLex, and although there are several leukocyte-bound structures that present SLex, it appears as though P-selectin must bind with PSGL-1 in order for leukocytes to efficiently roll along the endothelium under physiological flow conditions.	bind
37901	1	8743	5	13	NULL	NULL	NULL	AP-1	GP		bind					MMP-12	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_9_998_s_97	10807873	9  17 18  Both PMA and insulin increased the binding of AP-1 to the MMP-12 promoter, with higher affinity for the A allele (mean plus-or-minus SE, 57 plus-or-minus 37% [n=4] and 47 plus-or-minus 13% [n=3 higher binding affinity for the A probe than the G probe when stimulated with PMA or insulin, respectively) (Figures 3A   and 3B  ).	bind
37902	2	8743	5	13	NULL	NULL	NULL	PMA	Chemical		increase					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_9_998_s_97	10807873	9  17 18  Both PMA and insulin increased the binding of AP-1 to the MMP-12 promoter, with higher affinity for the A allele (mean plus-or-minus SE, 57 plus-or-minus 37% [n=4] and 47 plus-or-minus 13% [n=3 higher binding affinity for the A probe than the G probe when stimulated with PMA or insulin, respectively) (Figures 3A   and 3B  ).	bind
37903	3	8743	5	13	NULL	NULL	NULL	insulin	GP		increase					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_9_998_s_97	10807873	9  17 18  Both PMA and insulin increased the binding of AP-1 to the MMP-12 promoter, with higher affinity for the A allele (mean plus-or-minus SE, 57 plus-or-minus 37% [n=4] and 47 plus-or-minus 13% [n=3 higher binding affinity for the A probe than the G probe when stimulated with PMA or insulin, respectively) (Figures 3A   and 3B  ).	bind
37153	1	8743	7	NULL	NULL	0	NULL	AP-1	NULL		bind	NULL				MMP-12	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_circulationres_86_9_998_s_97	10807873	9  17 18  Both PMA and insulin increased the binding of AP-1 to the MMP-12 promoter, with higher affinity for the A allele (mean plus-or-minus SE, 57 plus-or-minus 37% [n=4] and 47 plus-or-minus 13% [n=3 higher binding affinity for the A probe than the G probe when stimulated with PMA or insulin, respectively) (Figures 3A   and 3B  ).	bind
37154	2	8743	7	NULL	NULL	0	NULL	PMA	NULL		increase	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_86_9_998_s_97	10807873	9  17 18  Both PMA and insulin increased the binding of AP-1 to the MMP-12 promoter, with higher affinity for the A allele (mean plus-or-minus SE, 57 plus-or-minus 37% [n=4] and 47 plus-or-minus 13% [n=3 higher binding affinity for the A probe than the G probe when stimulated with PMA or insulin, respectively) (Figures 3A   and 3B  ).	bind
37155	3	8743	7	NULL	NULL	0	NULL	insulin	NULL		increase	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_86_9_998_s_97	10807873	9  17 18  Both PMA and insulin increased the binding of AP-1 to the MMP-12 promoter, with higher affinity for the A allele (mean plus-or-minus SE, 57 plus-or-minus 37% [n=4] and 47 plus-or-minus 13% [n=3 higher binding affinity for the A probe than the G probe when stimulated with PMA or insulin, respectively) (Figures 3A   and 3B  ).	bind
37904	1	8744	5	13	NULL	NULL	NULL	Rab3A	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_163_3_889_s_170	12937130	9  Because the binding is inhibited by the GTP-bound form of Rab3A, the authors have hypothesized that, through switching the GTPase on and off and alternatively binding of rabphilin to Rab3A and alpha-actinin, these molecules behave like a timer that prepares vesicles for docking/fusion events by cytoskeletal reorganization.	bind
37905	2	8744	5	13	NULL	NULL	NULL	GTPase	GP	switching on	occurs simultaneously with					GTPase	GP	switching off			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_163_3_889_s_170	12937130	9  Because the binding is inhibited by the GTP-bound form of Rab3A, the authors have hypothesized that, through switching the GTPase on and off and alternatively binding of rabphilin to Rab3A and alpha-actinin, these molecules behave like a timer that prepares vesicles for docking/fusion events by cytoskeletal reorganization.	bind
37906	3	8744	5	13	NULL	NULL	NULL	rabphilin	GP		bind					Rab3A	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_163_3_889_s_170	12937130	9  Because the binding is inhibited by the GTP-bound form of Rab3A, the authors have hypothesized that, through switching the GTPase on and off and alternatively binding of rabphilin to Rab3A and alpha-actinin, these molecules behave like a timer that prepares vesicles for docking/fusion events by cytoskeletal reorganization.	bind
37907	4	8744	5	13	NULL	NULL	NULL	rabphilin	GP		bind					alpha-actinin	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_163_3_889_s_170	12937130	9  Because the binding is inhibited by the GTP-bound form of Rab3A, the authors have hypothesized that, through switching the GTPase on and off and alternatively binding of rabphilin to Rab3A and alpha-actinin, these molecules behave like a timer that prepares vesicles for docking/fusion events by cytoskeletal reorganization.	bind
37156	1	8744	7	NULL	NULL	0	NULL	 rabphilin	NULL		bind	NULL				Rab3A	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_163_3_889_s_170	12937130	9  Because the binding is inhibited by the GTP-bound form of Rab3A, the authors have hypothesized that, through switching the GTPase on and off and alternatively binding of rabphilin to Rab3A and alpha-actinin, these molecules behave like a timer that prepares vesicles for docking/fusion events by cytoskeletal reorganization.	bind
37157	2	8744	7	NULL	NULL	0	NULL	rabphilin	NULL		bind	NULL				alpha-actinin	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_163_3_889_s_170	12937130	9  Because the binding is inhibited by the GTP-bound form of Rab3A, the authors have hypothesized that, through switching the GTPase on and off and alternatively binding of rabphilin to Rab3A and alpha-actinin, these molecules behave like a timer that prepares vesicles for docking/fusion events by cytoskeletal reorganization.	bind
37160	4	8744	7	10	NULL	0	NULL	GTPase	NULL	switching on	occurs simultaneous with	NULL				GTPase	NULL	switching off			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_163_3_889_s_170	12937130	9  Because the binding is inhibited by the GTP-bound form of Rab3A, the authors have hypothesized that, through switching the GTPase on and off and alternatively binding of rabphilin to Rab3A and alpha-actinin, these molecules behave like a timer that prepares vesicles for docking/fusion events by cytoskeletal reorganization.	bind
46813	3	8744	7	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				Rab3A	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_163_3_889_s_170	12937130	9  Because the binding is inhibited by the GTP-bound form of Rab3A, the authors have hypothesized that, through switching the GTPase on and off and alternatively binding of rabphilin to Rab3A and alpha-actinin, these molecules behave like a timer that prepares vesicles for docking/fusion events by cytoskeletal reorganization.	bind
37923	1	8745	5	13	NULL	NULL	NULL	Fibronectin	GP		is a type of					ECM protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_5_1162_s_175	10323765	9  Fibronectin is another ECM protein that binds Lp(a).	bind
37924	2	8745	5	13	NULL	NULL	NULL	Fibronectin	GP		bind					Lp(a)	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_5_1162_s_175	10323765	9  Fibronectin is another ECM protein that binds Lp(a).	bind
37161	1	8745	7	NULL	NULL	0	NULL	Fibronectin	NULL		binds	NULL				Lp(a)	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_5_1162_s_175	10323765	9  Fibronectin is another ECM protein that binds Lp(a).	bind
37162	2	8745	7	NULL	NULL	0	NULL	fibronectin	NULL		is a type of	NULL				ECM protein	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_5_1162_s_175	10323765	9  Fibronectin is another ECM protein that binds Lp(a).	bind
37927	1	8746	5	10	NULL	0	NULL		NULL		associate with	NULL			KRE		NULL			KRE	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_8_937_s_202	10222341	9  KBF, by interfering with the self-association of KRE and/or the binding of HMG-1 and HMG-2, may abolish the silencer effect in GH3 cells (or heart).	bind
37928	2	8746	5	13	NULL	NULL	NULL	KBF	GP		interfere with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_8_937_s_202	10222341	9  KBF, by interfering with the self-association of KRE and/or the binding of HMG-1 and HMG-2, may abolish the silencer effect in GH3 cells (or heart).	bind
37929	3	8746	5	13	NULL	NULL	NULL	statement 2	Process		abolishes		may			silencer effect	Process				NULL	GH3 cells	NULL	NULL	NULL	NULL	gw60_circulationres_84_8_937_s_202	10222341	9  KBF, by interfering with the self-association of KRE and/or the binding of HMG-1 and HMG-2, may abolish the silencer effect in GH3 cells (or heart).	bind
37930	4	8746	5	13	NULL	NULL	NULL	statement 2	Process		abolishes		may			silencer effect	Process				NULL	heart	NULL	NULL	NULL	NULL	gw60_circulationres_84_8_937_s_202	10222341	9  KBF, by interfering with the self-association of KRE and/or the binding of HMG-1 and HMG-2, may abolish the silencer effect in GH3 cells (or heart).	bind
37931	5	8746	5	13	NULL	NULL	NULL	KBF	GP		interfere with					HMG-1	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_8_937_s_202	10222341	9  KBF, by interfering with the self-association of KRE and/or the binding of HMG-1 and HMG-2, may abolish the silencer effect in GH3 cells (or heart).	bind
37932	6	8746	5	13	NULL	NULL	NULL	KBF	GP		interfere with					HMG-2	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_8_937_s_202	10222341	9  KBF, by interfering with the self-association of KRE and/or the binding of HMG-1 and HMG-2, may abolish the silencer effect in GH3 cells (or heart).	bind
37933	7	8746	5	13	NULL	NULL	NULL	statement 5	Process		abolishes		may			silencer effect	Process				NULL	GH3 cells	NULL	NULL	NULL	NULL	gw60_circulationres_84_8_937_s_202	10222341	9  KBF, by interfering with the self-association of KRE and/or the binding of HMG-1 and HMG-2, may abolish the silencer effect in GH3 cells (or heart).	bind
37934	8	8746	5	13	NULL	NULL	NULL	statement 5	Process		abolishes		may			silencer effect	Process				NULL	heart	NULL	NULL	NULL	NULL	gw60_circulationres_84_8_937_s_202	10222341	9  KBF, by interfering with the self-association of KRE and/or the binding of HMG-1 and HMG-2, may abolish the silencer effect in GH3 cells (or heart).	bind
37935	9	8746	5	13	NULL	NULL	NULL	statement 6	Process		abolishes		may			silencer effect	Process				NULL	GH3 cells	NULL	NULL	NULL	NULL	gw60_circulationres_84_8_937_s_202	10222341	9  KBF, by interfering with the self-association of KRE and/or the binding of HMG-1 and HMG-2, may abolish the silencer effect in GH3 cells (or heart).	bind
37936	10	8746	5	13	NULL	NULL	NULL	statement 6	Process		abolishes		may			silencer effect	Process				NULL	heart	NULL	NULL	NULL	NULL	gw60_circulationres_84_8_937_s_202	10222341	9  KBF, by interfering with the self-association of KRE and/or the binding of HMG-1 and HMG-2, may abolish the silencer effect in GH3 cells (or heart).	bind
37163	1	8746	7	10	NULL	0	NULL	KRE			associates with					KRE					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_8_937_s_202	10222341	9  KBF, by interfering with the self-association of KRE and/or the binding of HMG-1 and HMG-2, may abolish the silencer effect in GH3 cells (or heart).	bind
37164	2	8746	7	10	NULL	0	NULL	KBF			interfers with					HMG-1		binding of 			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_8_937_s_202	10222341	9  KBF, by interfering with the self-association of KRE and/or the binding of HMG-1 and HMG-2, may abolish the silencer effect in GH3 cells (or heart).	bind
37165	3	8746	7	10	NULL	0	NULL	KBF			interfers with					HMG-2		binding of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_8_937_s_202	10222341	9  KBF, by interfering with the self-association of KRE and/or the binding of HMG-1 and HMG-2, may abolish the silencer effect in GH3 cells (or heart).	bind
37166	4	8746	7	10	NULL	0	NULL	statement 2			abolish		may			silencer effect					NULL	Heart	NULL	NULL	NULL	NULL	gw60_circulationres_84_8_937_s_202	10222341	9  KBF, by interfering with the self-association of KRE and/or the binding of HMG-1 and HMG-2, may abolish the silencer effect in GH3 cells (or heart).	bind
37167	5	8746	7	NULL	NULL	0	NULL	statement 2	NULL		abolish	NULL	may			silencer effect	NULL				NULL	GH3 cells	0	NULL	NULL	NULL	gw60_circulationres_84_8_937_s_202	10222341	9  KBF, by interfering with the self-association of KRE and/or the binding of HMG-1 and HMG-2, may abolish the silencer effect in GH3 cells (or heart).	bind
37168	6	8746	7	NULL	NULL	0	NULL	statement 3	NULL		abolish	NULL	may			silencer effect	NULL				NULL	GH3 cells	0	NULL	NULL	NULL	gw60_circulationres_84_8_937_s_202	10222341	9  KBF, by interfering with the self-association of KRE and/or the binding of HMG-1 and HMG-2, may abolish the silencer effect in GH3 cells (or heart).	bind
56359	7	8746	7	10	NULL	0	NULL	KBF			interfers with					statement 1					NULL		0	NULL	NULL	NULL	gw60_circulationres_84_8_937_s_202	10222341	9  KBF, by interfering with the self-association of KRE and/or the binding of HMG-1 and HMG-2, may abolish the silencer effect in GH3 cells (or heart).	bind
56360	8	8746	7	10	NULL	0	NULL	statement 3			abolish		may			silencer effect					NULL	Heart	0	NULL	NULL	NULL	gw60_circulationres_84_8_937_s_202	10222341	9  KBF, by interfering with the self-association of KRE and/or the binding of HMG-1 and HMG-2, may abolish the silencer effect in GH3 cells (or heart).	bind
56361	9	8746	7	10	NULL	0	NULL	statement 7			abolish		may			silencer effect					NULL	Heart	0	NULL	NULL	NULL	gw60_circulationres_84_8_937_s_202	10222341	9  KBF, by interfering with the self-association of KRE and/or the binding of HMG-1 and HMG-2, may abolish the silencer effect in GH3 cells (or heart).	bind
56362	8	8746	7	10	NULL	0	NULL	statement 7			abolish		may			silencer effect					NULL	GH3 cells	0	NULL	NULL	NULL	gw60_circulationres_84_8_937_s_202	10222341	9  KBF, by interfering with the self-association of KRE and/or the binding of HMG-1 and HMG-2, may abolish the silencer effect in GH3 cells (or heart).	bind
38000	1	8747	5	13	NULL	NULL	NULL	IgE antibodies	GP		bind					mast cells	Cell				NULL	lamina propria	NULL	NULL	NULL	NULL	gw60_amjpathol_158_2_681_s_28	11159205	9  Once in the lamina propria, antigen cross-links IgE antibodies bound to mast cells releasing mediators that act on epithelial receptors to induce ion secretion and enhance permeability of the paracellular pathway (both of which contribute to diarrhea).	bind
38001	2	8747	5	13	NULL	NULL	NULL	antigen	Chemical		cross-links					statement 1	Process				NULL	lamina propria	NULL	NULL	NULL	NULL	gw60_amjpathol_158_2_681_s_28	11159205	9  Once in the lamina propria, antigen cross-links IgE antibodies bound to mast cells releasing mediators that act on epithelial receptors to induce ion secretion and enhance permeability of the paracellular pathway (both of which contribute to diarrhea).	bind
38004	3	8747	5	13	NULL	NULL	NULL	statement 2	Process		release					mediators	GP				NULL	lamina propria	NULL	NULL	NULL	NULL	gw60_amjpathol_158_2_681_s_28	11159205	9  Once in the lamina propria, antigen cross-links IgE antibodies bound to mast cells releasing mediators that act on epithelial receptors to induce ion secretion and enhance permeability of the paracellular pathway (both of which contribute to diarrhea).	bind
38005	4	8747	5	13	NULL	NULL	NULL	mediators	GP		act on					epithelial receptors	GP				NULL	lamina propria	NULL	NULL	NULL	NULL	gw60_amjpathol_158_2_681_s_28	11159205	9  Once in the lamina propria, antigen cross-links IgE antibodies bound to mast cells releasing mediators that act on epithelial receptors to induce ion secretion and enhance permeability of the paracellular pathway (both of which contribute to diarrhea).	bind
38007	5	8747	5	13	NULL	NULL	NULL	statement 4	Process		induce					ion	Chemical	secretion of			NULL	lamina propria	NULL	NULL	NULL	NULL	gw60_amjpathol_158_2_681_s_28	11159205	9  Once in the lamina propria, antigen cross-links IgE antibodies bound to mast cells releasing mediators that act on epithelial receptors to induce ion secretion and enhance permeability of the paracellular pathway (both of which contribute to diarrhea).	bind
38008	6	8747	5	13	NULL	NULL	NULL	statement 4	Process		enhance					paracellular pathway	Process	permeability of			NULL	lamina propria	NULL	NULL	NULL	NULL	gw60_amjpathol_158_2_681_s_28	11159205	9  Once in the lamina propria, antigen cross-links IgE antibodies bound to mast cells releasing mediators that act on epithelial receptors to induce ion secretion and enhance permeability of the paracellular pathway (both of which contribute to diarrhea).	bind
38009	9	8747	5	13	NULL	NULL	NULL	statement 5	Process		contribute to					diarrhea	MedicalFinding				NULL	lamina propria	NULL	NULL	NULL	NULL	gw60_amjpathol_158_2_681_s_28	11159205	9  Once in the lamina propria, antigen cross-links IgE antibodies bound to mast cells releasing mediators that act on epithelial receptors to induce ion secretion and enhance permeability of the paracellular pathway (both of which contribute to diarrhea).	bind
38010	10	8747	5	13	NULL	NULL	NULL	statement 6	Process		contribute to					diarrhea	MedicalFinding				NULL	lamina propria	NULL	NULL	NULL	NULL	gw60_amjpathol_158_2_681_s_28	11159205	9  Once in the lamina propria, antigen cross-links IgE antibodies bound to mast cells releasing mediators that act on epithelial receptors to induce ion secretion and enhance permeability of the paracellular pathway (both of which contribute to diarrhea).	bind
37169	1	8747	7	NULL	NULL	0	NULL	IgE antibodies	NULL		bind	NULL				mast cells	NULL				NULL	lamina propria	0	NULL	NULL	NULL	gw60_amjpathol_158_2_681_s_28	11159205	9  Once in the lamina propria, antigen cross-links IgE antibodies bound to mast cells releasing mediators that act on epithelial receptors to induce ion secretion and enhance permeability of the paracellular pathway (both of which contribute to diarrhea).	bind
37170	2	8747	7	NULL	NULL	0	NULL	antigen	NULL		cross-links	NULL				statement 1	NULL				NULL	lamina propria	NULL	NULL	NULL	NULL	gw60_amjpathol_158_2_681_s_28	11159205	9  Once in the lamina propria, antigen cross-links IgE antibodies bound to mast cells releasing mediators that act on epithelial receptors to induce ion secretion and enhance permeability of the paracellular pathway (both of which contribute to diarrhea).	bind
37171	3	8747	7	NULL	NULL	0	NULL	statement 1	NULL		release	NULL				mediators	NULL				NULL	lamina propria	NULL	NULL	NULL	NULL	gw60_amjpathol_158_2_681_s_28	11159205	9  Once in the lamina propria, antigen cross-links IgE antibodies bound to mast cells releasing mediators that act on epithelial receptors to induce ion secretion and enhance permeability of the paracellular pathway (both of which contribute to diarrhea).	bind
37172	4	8747	7	NULL	NULL	0	NULL	mediators	NULL		act on	NULL				epithelial receptors	NULL				NULL	lamina propria	NULL	NULL	NULL	NULL	gw60_amjpathol_158_2_681_s_28	11159205	9  Once in the lamina propria, antigen cross-links IgE antibodies bound to mast cells releasing mediators that act on epithelial receptors to induce ion secretion and enhance permeability of the paracellular pathway (both of which contribute to diarrhea).	bind
37173	5	8747	7	10	NULL	0	NULL	statement 4			induce					ion		secretion of 			NULL	lamina propria	NULL	NULL	NULL	NULL	gw60_amjpathol_158_2_681_s_28	11159205	9  Once in the lamina propria, antigen cross-links IgE antibodies bound to mast cells releasing mediators that act on epithelial receptors to induce ion secretion and enhance permeability of the paracellular pathway (both of which contribute to diarrhea).	bind
37174	6	8747	7	10	NULL	0	NULL	statement 4			enhance					paracellular pathway		permeabilty of 			NULL	lamina propria	NULL	NULL	NULL	NULL	gw60_amjpathol_158_2_681_s_28	11159205	9  Once in the lamina propria, antigen cross-links IgE antibodies bound to mast cells releasing mediators that act on epithelial receptors to induce ion secretion and enhance permeability of the paracellular pathway (both of which contribute to diarrhea).	bind
37175	7	8747	7	NULL	NULL	0	NULL	statement 5	NULL		contribute to	NULL				diarrhea	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_2_681_s_28	11159205	9  Once in the lamina propria, antigen cross-links IgE antibodies bound to mast cells releasing mediators that act on epithelial receptors to induce ion secretion and enhance permeability of the paracellular pathway (both of which contribute to diarrhea).	bind
37176	8	8747	7	NULL	NULL	0	NULL	statement 6	NULL		contribute to	NULL				diarrhea	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_158_2_681_s_28	11159205	9  Once in the lamina propria, antigen cross-links IgE antibodies bound to mast cells releasing mediators that act on epithelial receptors to induce ion secretion and enhance permeability of the paracellular pathway (both of which contribute to diarrhea).	bind
38020	1	8748	5	13	NULL	NULL	NULL	Raf	GP	activation of	mediated by					H-Ras	GP				NULL	hamster kidney cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_11_2465_s_209	11073854	9  Recently, Roy et al 26  reported that in hamster kidney cells, dominant-negative caveolin-3 completely blocked Raf activation mediated by H-Ras, and the inhibitory effect was reversed by replenishing cell membranes with cholesterol.	bind
38021	2	8748	5	13	NULL	NULL	NULL	caveolin-3	GP	dominant-negative	block		completely			statement 1	Process				NULL	hamster kidney cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_11_2465_s_209	11073854	9  Recently, Roy et al 26  reported that in hamster kidney cells, dominant-negative caveolin-3 completely blocked Raf activation mediated by H-Ras, and the inhibitory effect was reversed by replenishing cell membranes with cholesterol.	bind
38023	3	8748	5	13	NULL	NULL	NULL	cell membranes	CellComponent		is replenished with					cholesterol	Chemical				NULL	hamster kidney cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_11_2465_s_209	11073854	9  Recently, Roy et al 26  reported that in hamster kidney cells, dominant-negative caveolin-3 completely blocked Raf activation mediated by H-Ras, and the inhibitory effect was reversed by replenishing cell membranes with cholesterol.	bind
38024	4	8748	5	13	NULL	NULL	NULL	statement 2	Process	inhibitory effect of	is reversed by					statement 3	Process				NULL	hamster kidney cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_11_2465_s_209	11073854	9  Recently, Roy et al 26  reported that in hamster kidney cells, dominant-negative caveolin-3 completely blocked Raf activation mediated by H-Ras, and the inhibitory effect was reversed by replenishing cell membranes with cholesterol.	bind
37177	1	8748	7	NULL	NULL	0	NULL	H-Ras	NULL		mediate	NULL				Raf	NULL	activation of			NULL	hamster kidney cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_11_2465_s_209	11073854	9  Recently, Roy et al 26  reported that in hamster kidney cells, dominant-negative caveolin-3 completely blocked Raf activation mediated by H-Ras, and the inhibitory effect was reversed by replenishing cell membranes with cholesterol.	bind
37178	2	8748	7	10	NULL	0	NULL	caveolin-3	NULL	dominant-negative 	blocks	NULL	completely			statement 1	NULL				NULL	hamster kidney cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_11_2465_s_209	11073854	9  Recently, Roy et al 26  reported that in hamster kidney cells, dominant-negative caveolin-3 completely blocked Raf activation mediated by H-Ras, and the inhibitory effect was reversed by replenishing cell membranes with cholesterol.	bind
37179	3	8748	7	NULL	NULL	0	NULL	cell membranes	NULL		replenished with	NULL				cholesterol	NULL				NULL	hamster kidney cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_11_2465_s_209	11073854	9  Recently, Roy et al 26  reported that in hamster kidney cells, dominant-negative caveolin-3 completely blocked Raf activation mediated by H-Ras, and the inhibitory effect was reversed by replenishing cell membranes with cholesterol.	bind
37180	4	8748	7	10	NULL	0	NULL	statement 2	NULL	inhibitory effect of 	reversed by	NULL				statement 3	NULL				NULL	hamster kidney cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_11_2465_s_209	11073854	9  Recently, Roy et al 26  reported that in hamster kidney cells, dominant-negative caveolin-3 completely blocked Raf activation mediated by H-Ras, and the inhibitory effect was reversed by replenishing cell membranes with cholesterol.	bind
38068	1	8749	5	13	NULL	NULL	NULL	CREB	GP		is					cAMP-responsive element - binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_7_805_s_23	10683356	9  The cyclin A promoter contains activating transcription factor (ATF) or cAMP-responsive element (CRE), which are bound by cAMP-responsive element - binding protein (CREB) and ATF-1 by heterodimer formation.	bind
38069	2	8749	5	13	NULL	NULL	NULL	CREB	GP		bind					ATF-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_7_805_s_23	10683356	9  The cyclin A promoter contains activating transcription factor (ATF) or cAMP-responsive element (CRE), which are bound by cAMP-responsive element - binding protein (CREB) and ATF-1 by heterodimer formation.	bind
38070	4	8749	5	13	NULL	NULL	NULL	statement 3	GP		bind					cyclin A	GP			ATF site in promoter	NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_7_805_s_23	10683356	9  The cyclin A promoter contains activating transcription factor (ATF) or cAMP-responsive element (CRE), which are bound by cAMP-responsive element - binding protein (CREB) and ATF-1 by heterodimer formation.	bind
38071	5	8749	5	13	NULL	NULL	NULL	statement 3	GP		bind					cyclin A	GP			CRE in promoter	NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_7_805_s_23	10683356	9  The cyclin A promoter contains activating transcription factor (ATF) or cAMP-responsive element (CRE), which are bound by cAMP-responsive element - binding protein (CREB) and ATF-1 by heterodimer formation.	bind
38072	6	8749	5	13	NULL	NULL	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_7_805_s_23	10683356	9  The cyclin A promoter contains activating transcription factor (ATF) or cAMP-responsive element (CRE), which are bound by cAMP-responsive element - binding protein (CREB) and ATF-1 by heterodimer formation.	bind
38073	7	8749	5	13	NULL	NULL	NULL	CRE	GP		is					cAMP-responsive element	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_7_805_s_23	10683356	9  The cyclin A promoter contains activating transcription factor (ATF) or cAMP-responsive element (CRE), which are bound by cAMP-responsive element - binding protein (CREB) and ATF-1 by heterodimer formation.	bind
38074	8	8749	5	13	NULL	NULL	NULL	ATF	GP		is					activating transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_7_805_s_23	10683356	9  The cyclin A promoter contains activating transcription factor (ATF) or cAMP-responsive element (CRE), which are bound by cAMP-responsive element - binding protein (CREB) and ATF-1 by heterodimer formation.	bind
38075	3	8749	5	13	NULL	NULL	NULL	statement 2	GP		forms					CREB/ATF-1 heterodimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_7_805_s_23	10683356	9  The cyclin A promoter contains activating transcription factor (ATF) or cAMP-responsive element (CRE), which are bound by cAMP-responsive element - binding protein (CREB) and ATF-1 by heterodimer formation.	bind
37181	1	8749	7	10	NULL	0	NULL	cyclin A 			contains					ATF					NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_7_805_s_23	10683356	9  The cyclin A promoter contains activating transcription factor (ATF) or cAMP-responsive element (CRE), which are bound by cAMP-responsive element - binding protein (CREB) and ATF-1 by heterodimer formation.	bind
37182	2	8749	7	10	NULL	0	NULL	cyclin A			contains					CRE					NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_7_805_s_23	10683356	9  The cyclin A promoter contains activating transcription factor (ATF) or cAMP-responsive element (CRE), which are bound by cAMP-responsive element - binding protein (CREB) and ATF-1 by heterodimer formation.	bind
37183	3	8749	7	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_7_805_s_23	10683356	9  The cyclin A promoter contains activating transcription factor (ATF) or cAMP-responsive element (CRE), which are bound by cAMP-responsive element - binding protein (CREB) and ATF-1 by heterodimer formation.	bind
37184	4	8749	7	NULL	NULL	0	NULL	CREB	NULL		heterodimerizes with	NULL				ATF1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_101_7_805_s_23	10683356	9  The cyclin A promoter contains activating transcription factor (ATF) or cAMP-responsive element (CRE), which are bound by cAMP-responsive element - binding protein (CREB) and ATF-1 by heterodimer formation.	bind
37185	5	8749	7	NULL	NULL	0	NULL	statement 4	NULL		bind	NULL				cyclin A	NULL			ATF	NULL		0	NULL	NULL	NULL	gw60_circulation_101_7_805_s_23	10683356	9  The cyclin A promoter contains activating transcription factor (ATF) or cAMP-responsive element (CRE), which are bound by cAMP-responsive element - binding protein (CREB) and ATF-1 by heterodimer formation.	bind
37186	6	8749	7	NULL	NULL	0	NULL	statement 4	NULL		bind	NULL				cyclin A	NULL			CRE	NULL		0	NULL	NULL	NULL	gw60_circulation_101_7_805_s_23	10683356	9  The cyclin A promoter contains activating transcription factor (ATF) or cAMP-responsive element (CRE), which are bound by cAMP-responsive element - binding protein (CREB) and ATF-1 by heterodimer formation.	bind
37187	7	8749	7	NULL	NULL	0	NULL	ATF	NULL		is	NULL				activating transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_101_7_805_s_23	10683356	9  The cyclin A promoter contains activating transcription factor (ATF) or cAMP-responsive element (CRE), which are bound by cAMP-responsive element - binding protein (CREB) and ATF-1 by heterodimer formation.	bind
37188	8	8749	7	NULL	NULL	0	NULL	CRE	NULL		is	NULL				cAMP-responsive element 	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_101_7_805_s_23	10683356	9  The cyclin A promoter contains activating transcription factor (ATF) or cAMP-responsive element (CRE), which are bound by cAMP-responsive element - binding protein (CREB) and ATF-1 by heterodimer formation.	bind
37189	9	8749	7	NULL	NULL	0	NULL	CREB	NULL		is	NULL				cAMP-responsive element - binding protein	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_101_7_805_s_23	10683356	9  The cyclin A promoter contains activating transcription factor (ATF) or cAMP-responsive element (CRE), which are bound by cAMP-responsive element - binding protein (CREB) and ATF-1 by heterodimer formation.	bind
38076	1	8750	5	13	NULL	NULL	NULL	VASP	GP		bind			tandem repeat of 3 GP5 motifs		profilin	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2051_s_28	10978248	9  VASP binds profilin, zyxin, vinculin, and the bacterial coat protein ActA. 10 11 12  13  Binding of the G-actin binding protein profilin is likely to be mediated by the tandem repeat of 3 GP5 motifs within VASP. 11  14 15 16  The amino-terminal EVH-1 domain of VASP is responsible for binding ActA as well as the adhesion proteins zyxin and vinculin.	bind
38077	2	8750	5	13	NULL	NULL	NULL	VASP	GP		bind			amino-terminal EVH-1 domain		zyxin	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2051_s_28	10978248	9  VASP binds profilin, zyxin, vinculin, and the bacterial coat protein ActA. 10 11 12  13  Binding of the G-actin binding protein profilin is likely to be mediated by the tandem repeat of 3 GP5 motifs within VASP. 11  14 15 16  The amino-terminal EVH-1 domain of VASP is responsible for binding ActA as well as the adhesion proteins zyxin and vinculin.	bind
38078	3	8750	5	13	NULL	NULL	NULL	VASP	GP		bind			amino-terminal EVH-1 domain		vinculin	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2051_s_28	10978248	9  VASP binds profilin, zyxin, vinculin, and the bacterial coat protein ActA. 10 11 12  13  Binding of the G-actin binding protein profilin is likely to be mediated by the tandem repeat of 3 GP5 motifs within VASP. 11  14 15 16  The amino-terminal EVH-1 domain of VASP is responsible for binding ActA as well as the adhesion proteins zyxin and vinculin.	bind
38079	4	8750	5	13	NULL	NULL	NULL	VASP	GP		bind			amino-terminal EVH-1 domain		ActA	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2051_s_28	10978248	9  VASP binds profilin, zyxin, vinculin, and the bacterial coat protein ActA. 10 11 12  13  Binding of the G-actin binding protein profilin is likely to be mediated by the tandem repeat of 3 GP5 motifs within VASP. 11  14 15 16  The amino-terminal EVH-1 domain of VASP is responsible for binding ActA as well as the adhesion proteins zyxin and vinculin.	bind
38080	5	8750	5	13	NULL	NULL	NULL	ActA	GP		is a type of					bacterial coat protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2051_s_28	10978248	9  VASP binds profilin, zyxin, vinculin, and the bacterial coat protein ActA. 10 11 12  13  Binding of the G-actin binding protein profilin is likely to be mediated by the tandem repeat of 3 GP5 motifs within VASP. 11  14 15 16  The amino-terminal EVH-1 domain of VASP is responsible for binding ActA as well as the adhesion proteins zyxin and vinculin.	bind
38081	6	8750	5	13	NULL	NULL	NULL	profilin	GP		is a type of					G-actin binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2051_s_28	10978248	9  VASP binds profilin, zyxin, vinculin, and the bacterial coat protein ActA. 10 11 12  13  Binding of the G-actin binding protein profilin is likely to be mediated by the tandem repeat of 3 GP5 motifs within VASP. 11  14 15 16  The amino-terminal EVH-1 domain of VASP is responsible for binding ActA as well as the adhesion proteins zyxin and vinculin.	bind
38082	7	8750	5	13	NULL	NULL	NULL	zyxin	GP		is a type of					adhesion proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2051_s_28	10978248	9  VASP binds profilin, zyxin, vinculin, and the bacterial coat protein ActA. 10 11 12  13  Binding of the G-actin binding protein profilin is likely to be mediated by the tandem repeat of 3 GP5 motifs within VASP. 11  14 15 16  The amino-terminal EVH-1 domain of VASP is responsible for binding ActA as well as the adhesion proteins zyxin and vinculin.	bind
38083	8	8750	5	13	NULL	NULL	NULL	vinculin	GP		is a type of					adhesion proteins					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2051_s_28	10978248	9  VASP binds profilin, zyxin, vinculin, and the bacterial coat protein ActA. 10 11 12  13  Binding of the G-actin binding protein profilin is likely to be mediated by the tandem repeat of 3 GP5 motifs within VASP. 11  14 15 16  The amino-terminal EVH-1 domain of VASP is responsible for binding ActA as well as the adhesion proteins zyxin and vinculin.	bind
37190	1	8750	7	NULL	NULL	0	NULL	VASP	NULL		binds	NULL				profilin	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2051_s_28	10978248	9  VASP binds profilin, zyxin, vinculin, and the bacterial coat protein ActA. 10 11 12  13  Binding of the G-actin binding protein profilin is likely to be mediated by the tandem repeat of 3 GP5 motifs within VASP. 11  14 15 16  The amino-terminal EVH-1 domain of VASP is responsible for binding ActA as well as the adhesion proteins zyxin and vinculin.	bind
37191	2	8750	7	NULL	NULL	0	NULL	VASP	NULL		binds	NULL		amino-terminal EVH-1 domain		zyxin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2051_s_28	10978248	9  VASP binds profilin, zyxin, vinculin, and the bacterial coat protein ActA. 10 11 12  13  Binding of the G-actin binding protein profilin is likely to be mediated by the tandem repeat of 3 GP5 motifs within VASP. 11  14 15 16  The amino-terminal EVH-1 domain of VASP is responsible for binding ActA as well as the adhesion proteins zyxin and vinculin.	bind
37192	3	8750	7	NULL	NULL	0	NULL	VASP	NULL		binds	NULL		amino-terminal EVH-1 domain		vinculin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2051_s_28	10978248	9  VASP binds profilin, zyxin, vinculin, and the bacterial coat protein ActA. 10 11 12  13  Binding of the G-actin binding protein profilin is likely to be mediated by the tandem repeat of 3 GP5 motifs within VASP. 11  14 15 16  The amino-terminal EVH-1 domain of VASP is responsible for binding ActA as well as the adhesion proteins zyxin and vinculin.	bind
37193	4	8750	7	NULL	NULL	0	NULL	VASP	NULL		binds	NULL		amino-terminal EVH-1 domain		ActA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2051_s_28	10978248	9  VASP binds profilin, zyxin, vinculin, and the bacterial coat protein ActA. 10 11 12  13  Binding of the G-actin binding protein profilin is likely to be mediated by the tandem repeat of 3 GP5 motifs within VASP. 11  14 15 16  The amino-terminal EVH-1 domain of VASP is responsible for binding ActA as well as the adhesion proteins zyxin and vinculin.	bind
37194	5	8750	7	NULL	NULL	0	NULL	VASP	NULL		mediates	NULL		tandem repeat of 3 GP5 motifs		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2051_s_28	10978248	9  VASP binds profilin, zyxin, vinculin, and the bacterial coat protein ActA. 10 11 12  13  Binding of the G-actin binding protein profilin is likely to be mediated by the tandem repeat of 3 GP5 motifs within VASP. 11  14 15 16  The amino-terminal EVH-1 domain of VASP is responsible for binding ActA as well as the adhesion proteins zyxin and vinculin.	bind
37195	6	8750	7	NULL	NULL	0	NULL	ActA	NULL		is a type of	NULL				bacterial coat protein	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2051_s_28	10978248	9  VASP binds profilin, zyxin, vinculin, and the bacterial coat protein ActA. 10 11 12  13  Binding of the G-actin binding protein profilin is likely to be mediated by the tandem repeat of 3 GP5 motifs within VASP. 11  14 15 16  The amino-terminal EVH-1 domain of VASP is responsible for binding ActA as well as the adhesion proteins zyxin and vinculin.	bind
37196	7	8750	7	NULL	NULL	0	NULL	profilin	NULL		is a type of	NULL				G-actin binding protein	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2051_s_28	10978248	9  VASP binds profilin, zyxin, vinculin, and the bacterial coat protein ActA. 10 11 12  13  Binding of the G-actin binding protein profilin is likely to be mediated by the tandem repeat of 3 GP5 motifs within VASP. 11  14 15 16  The amino-terminal EVH-1 domain of VASP is responsible for binding ActA as well as the adhesion proteins zyxin and vinculin.	bind
37197	8	8750	7	NULL	NULL	0	NULL	zyxin	NULL		is a type of	NULL				adhesion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2051_s_28	10978248	9  VASP binds profilin, zyxin, vinculin, and the bacterial coat protein ActA. 10 11 12  13  Binding of the G-actin binding protein profilin is likely to be mediated by the tandem repeat of 3 GP5 motifs within VASP. 11  14 15 16  The amino-terminal EVH-1 domain of VASP is responsible for binding ActA as well as the adhesion proteins zyxin and vinculin.	bind
37198	9	8750	7	NULL	NULL	0	NULL	vinculin	NULL		is a type of	NULL				adhesion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_9_2051_s_28	10978248	9  VASP binds profilin, zyxin, vinculin, and the bacterial coat protein ActA. 10 11 12  13  Binding of the G-actin binding protein profilin is likely to be mediated by the tandem repeat of 3 GP5 motifs within VASP. 11  14 15 16  The amino-terminal EVH-1 domain of VASP is responsible for binding ActA as well as the adhesion proteins zyxin and vinculin.	bind
38084	1	8751	5	13	NULL	NULL	NULL	LDL	GP		bind					GAGs	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_12_1902_s_15	11742862	9 -  11 Most important, Boren et al 12 have shown that despite hypercholesterolemia, the development of atherosclerotic lesions is delayed in mice expressing proteoglycan-binding-deficient LDL, suggesting that binding of LDL to GAGs has a causal role in the development of atherosclerosis.	bind
38085	2	8751	5	13	NULL	NULL	NULL	statement 1	Process		plays a role in					atherosclerosis	MedicalFinding	development of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_12_1902_s_15	11742862	9 -  11 Most important, Boren et al 12 have shown that despite hypercholesterolemia, the development of atherosclerotic lesions is delayed in mice expressing proteoglycan-binding-deficient LDL, suggesting that binding of LDL to GAGs has a causal role in the development of atherosclerosis.	bind
37199	1	8751	7	NULL	NULL	0	NULL	LDL	NULL		bind	NULL				GAGs	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_12_1902_s_15	11742862	9 -  11 Most important, Boren et al 12 have shown that despite hypercholesterolemia, the development of atherosclerotic lesions is delayed in mice expressing proteoglycan-binding-deficient LDL, suggesting that binding of LDL to GAGs has a causal role in the development of atherosclerosis.	bind
37200	2	8751	7	10	NULL	0	NULL	statement 1	NULL		plays a role in	NULL				atherosclerosis	NULL	development of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_21_12_1902_s_15	11742862	9 -  11 Most important, Boren et al 12 have shown that despite hypercholesterolemia, the development of atherosclerotic lesions is delayed in mice expressing proteoglycan-binding-deficient LDL, suggesting that binding of LDL to GAGs has a causal role in the development of atherosclerosis.	bind
38089	1	8752	5	13	NULL	NULL	NULL	Gab1	GP	mutant	does not bind					SHP2	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulationres_93_3_221_s_26	12855672	9 - 12    The functional significance of Gab1-SHP2 interaction has been extensively studied using mutants of Gab1 unable to bind SHP2 in vitro and in vivo.	bind
38090	2	8752	5	13	NULL	NULL	NULL	Gab1	GP	mutant	does not bind					SHP2	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_circulationres_93_3_221_s_26	12855672	9 - 12    The functional significance of Gab1-SHP2 interaction has been extensively studied using mutants of Gab1 unable to bind SHP2 in vitro and in vivo.	bind
37202	1	8752	7	10	NULL	0	NULL	Gab1		mutant	does not bind					SHP2					NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulationres_93_3_221_s_26	12855672	9 - 12    The functional significance of Gab1-SHP2 interaction has been extensively studied using mutants of Gab1 unable to bind SHP2 in vitro and in vivo.	bind
56363	2	8752	7	10	NULL	0	NULL	Gab1		mutant	does not bind					SHP2					NULL	in vivo	0	NULL	NULL	NULL	gw60_circulationres_93_3_221_s_26	12855672	9 - 12    The functional significance of Gab1-SHP2 interaction has been extensively studied using mutants of Gab1 unable to bind SHP2 in vitro and in vivo.	bind
38091	1	8753	5	13	NULL	NULL	NULL	vWF	GP		bind					GP Ib/IX	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_10_3281_s_24	9396417	9 - 14 It is now believed that binding of vWF to GP Ib/IX initiates intracellular signals resulting in activation of another platelet receptor, GP IIb/IIa complex, to form platelet clumps.	bind
38092	2	8753	5	13	NULL	NULL	NULL	statement 1	Process		initiate					intracellular signals	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_10_3281_s_24	9396417	9 - 14 It is now believed that binding of vWF to GP Ib/IX initiates intracellular signals resulting in activation of another platelet receptor, GP IIb/IIa complex, to form platelet clumps.	bind
38093	3	8753	5	13	NULL	NULL	NULL	statement 2	Process		activates					GP IIb/IIa complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_10_3281_s_24	9396417	9 - 14 It is now believed that binding of vWF to GP Ib/IX initiates intracellular signals resulting in activation of another platelet receptor, GP IIb/IIa complex, to form platelet clumps.	bind
38094	4	8753	5	13	NULL	NULL	NULL	GP IIb/IIa complex	GP		is a type of					platelet receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_10_3281_s_24	9396417	9 - 14 It is now believed that binding of vWF to GP Ib/IX initiates intracellular signals resulting in activation of another platelet receptor, GP IIb/IIa complex, to form platelet clumps.	bind
38095	5	8753	5	13	NULL	NULL	NULL	statement 3	Process		forms					platelet clumps	Cell				NULL		NULL	NULL	NULL	NULL	gw60_circulation_96_10_3281_s_24	9396417	9 - 14 It is now believed that binding of vWF to GP Ib/IX initiates intracellular signals resulting in activation of another platelet receptor, GP IIb/IIa complex, to form platelet clumps.	bind
37204	1	8753	7	NULL	NULL	0	NULL	vWF	NULL		bind	NULL				GP Ib/IX	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_96_10_3281_s_24	9396417	9 - 14 It is now believed that binding of vWF to GP Ib/IX initiates intracellular signals resulting in activation of another platelet receptor, GP IIb/IIa complex, to form platelet clumps.	bind
37205	2	8753	7	NULL	NULL	0	NULL	statement 1	NULL		initiates	NULL				intracellular signals	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_96_10_3281_s_24	9396417	9 - 14 It is now believed that binding of vWF to GP Ib/IX initiates intracellular signals resulting in activation of another platelet receptor, GP IIb/IIa complex, to form platelet clumps.	bind
37206	3	8753	7	NULL	NULL	0	NULL	statement 2	NULL		results in	NULL				GP IIb/IIa complex	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_circulation_96_10_3281_s_24	9396417	9 - 14 It is now believed that binding of vWF to GP Ib/IX initiates intracellular signals resulting in activation of another platelet receptor, GP IIb/IIa complex, to form platelet clumps.	bind
37207	4	8753	7	NULL	NULL	0	NULL	statement 3	NULL		form	NULL				platelet clumps	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_96_10_3281_s_24	9396417	9 - 14 It is now believed that binding of vWF to GP Ib/IX initiates intracellular signals resulting in activation of another platelet receptor, GP IIb/IIa complex, to form platelet clumps.	bind
37208	5	8753	7	NULL	NULL	0	NULL	GP IIb/IIa complex	NULL		is a type of	NULL				platelet receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_96_10_3281_s_24	9396417	9 - 14 It is now believed that binding of vWF to GP Ib/IX initiates intracellular signals resulting in activation of another platelet receptor, GP IIb/IIa complex, to form platelet clumps.	bind
38096	1	8754	5	13	NULL	NULL	NULL	VEGF-B	GP		bind					VEGFR-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_18_2262_s_34	11056103	9 10  Other members of the VEGF family have also been characterized: VEGF-B 11  binds to VEGFR-1, and VEGF-D 12  binds to VEGFR-2 and VEGFR-3.	bind
38097	2	8754	5	13	NULL	NULL	NULL	VEGF-D	GP		bind					VEGFR-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_18_2262_s_34	11056103	9 10  Other members of the VEGF family have also been characterized: VEGF-B 11  binds to VEGFR-1, and VEGF-D 12  binds to VEGFR-2 and VEGFR-3.	bind
38098	3	8754	5	13	NULL	NULL	NULL	VEGF-D	GP		bind					VEGFR-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_18_2262_s_34	11056103	9 10  Other members of the VEGF family have also been characterized: VEGF-B 11  binds to VEGFR-1, and VEGF-D 12  binds to VEGFR-2 and VEGFR-3.	bind
37209	1	8754	7	10	NULL	0	NULL	VEGF-B	NULL		binds to	NULL				VEGFR-1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_18_2262_s_34	11056103	9 10  Other members of the VEGF family have also been characterized: VEGF-B 11  binds to VEGFR-1, and VEGF-D 12  binds to VEGFR-2 and VEGFR-3.	bind
37210	2	8754	7	10	NULL	0	NULL	 VEGF-D	NULL		binds to	NULL				VEGFR-2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_18_2262_s_34	11056103	9 10  Other members of the VEGF family have also been characterized: VEGF-B 11  binds to VEGFR-1, and VEGF-D 12  binds to VEGFR-2 and VEGFR-3.	bind
37211	3	8754	7	10	NULL	0	NULL	 VEGF-D	NULL		binds to	NULL				VEGFR-3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_18_2262_s_34	11056103	9 10  Other members of the VEGF family have also been characterized: VEGF-B 11  binds to VEGFR-1, and VEGF-D 12  binds to VEGFR-2 and VEGFR-3.	bind
38113	1	8755	5	13	NULL	NULL	NULL	p47 phox	GP		bind			second SH3 domain		p67 phox	GP		proline-rich region		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_12_1195_s_202	11110778	9 10  The second SH3 domain of p47 phox binds to the proline-rich region of p67 phox, and the N-terminal half of p67 phox contains a binding region for Rac.	bind
38114	2	8755	5	13	NULL	NULL	NULL	p67 phox	GP		contains			N-terminal half					binding region for Rac		NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_12_1195_s_202	11110778	9 10  The second SH3 domain of p47 phox binds to the proline-rich region of p67 phox, and the N-terminal half of p67 phox contains a binding region for Rac.	bind
37212	1	8755	7	NULL	NULL	0	NULL	p47 phox 	NULL		binds to	NULL		second SH3 domain		 p67 phox	NULL		proline-rich region		NULL		0	NULL	NULL	NULL	gw60_circulationres_87_12_1195_s_202	11110778	9 10  The second SH3 domain of p47 phox binds to the proline-rich region of p67 phox, and the N-terminal half of p67 phox contains a binding region for Rac.	bind
37213	2	8755	7	NULL	NULL	0	NULL	p67 phox	NULL		contains	NULL		 N-terminal half of		Rac	NULL		binding region 		NULL		0	NULL	NULL	NULL	gw60_circulationres_87_12_1195_s_202	11110778	9 10  The second SH3 domain of p47 phox binds to the proline-rich region of p67 phox, and the N-terminal half of p67 phox contains a binding region for Rac.	bind
38107	1	8756	5	13	NULL	NULL	NULL	VEGF-C	GP		bind					VEGFR-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_18_2262_s_33	11056103	9 10  VEGF-C binds to VEGFR-2 and VEGFR-3 and has been shown to stimulate both angiogenesis and formation of lymphatic vessels.	bind
38108	2	8756	5	13	NULL	NULL	NULL	VEGF-C	GP		bind					VEGFR-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_18_2262_s_33	11056103	9 10  VEGF-C binds to VEGFR-2 and VEGFR-3 and has been shown to stimulate both angiogenesis and formation of lymphatic vessels.	bind
38109	3	8756	5	13	NULL	NULL	NULL	statement 1	Process		stimulate					angiogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_18_2262_s_33	11056103	9 10  VEGF-C binds to VEGFR-2 and VEGFR-3 and has been shown to stimulate both angiogenesis and formation of lymphatic vessels.	bind
38110	4	8756	5	13	NULL	NULL	NULL	statement 2	Process		stimulate					angiogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_18_2262_s_33	11056103	9 10  VEGF-C binds to VEGFR-2 and VEGFR-3 and has been shown to stimulate both angiogenesis and formation of lymphatic vessels.	bind
38111	5	8756	5	13	NULL	NULL	NULL	statement 1	Process		stimulate					lymphatic vessels	OrganismPart	formation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_18_2262_s_33	11056103	9 10  VEGF-C binds to VEGFR-2 and VEGFR-3 and has been shown to stimulate both angiogenesis and formation of lymphatic vessels.	bind
38112	6	8756	5	13	NULL	NULL	NULL	statement 2	Process		stimulate					lymphatic vessels	OrganismPart	formation of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_18_2262_s_33	11056103	9 10  VEGF-C binds to VEGFR-2 and VEGFR-3 and has been shown to stimulate both angiogenesis and formation of lymphatic vessels.	bind
37353	1	8756	7	NULL	NULL	0	NULL	VEGF-C	NULL		binds to	NULL				VEGFR-2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_102_18_2262_s_33	11056103	9 10  VEGF-C binds to VEGFR-2 and VEGFR-3 and has been shown to stimulate both angiogenesis and formation of lymphatic vessels.	bind
37354	2	8756	7	NULL	NULL	0	NULL	VEGF-C	NULL		binds to	NULL				VEGFR-3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_102_18_2262_s_33	11056103	9 10  VEGF-C binds to VEGFR-2 and VEGFR-3 and has been shown to stimulate both angiogenesis and formation of lymphatic vessels.	bind
37355	3	8756	7	NULL	NULL	0	NULL	statement 1	NULL		stimulate	NULL				angiogenesis	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_102_18_2262_s_33	11056103	9 10  VEGF-C binds to VEGFR-2 and VEGFR-3 and has been shown to stimulate both angiogenesis and formation of lymphatic vessels.	bind
37356	4	8756	7	NULL	NULL	0	NULL	statement 2	NULL		stimulate	NULL				angiogenesis	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_102_18_2262_s_33	11056103	9 10  VEGF-C binds to VEGFR-2 and VEGFR-3 and has been shown to stimulate both angiogenesis and formation of lymphatic vessels.	bind
37357	5	8756	7	NULL	NULL	0	NULL	statement 1	NULL		stimulate	NULL				lymphatic vessels	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_circulation_102_18_2262_s_33	11056103	9 10  VEGF-C binds to VEGFR-2 and VEGFR-3 and has been shown to stimulate both angiogenesis and formation of lymphatic vessels.	bind
37358	6	8756	7	NULL	NULL	0	NULL	statement 2	NULL		stimulate	NULL				lymphatic vessels	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_circulation_102_18_2262_s_33	11056103	9 10  VEGF-C binds to VEGFR-2 and VEGFR-3 and has been shown to stimulate both angiogenesis and formation of lymphatic vessels.	bind
38104	1	8757	5	13	NULL	NULL	NULL	SMCs	Cell		express					IAP	GP				NULL	cell surface	NULL	NULL	NULL	NULL	gw70_circulationres_93_10_925_s_62	14563713	9 Because we have also determined that SMCs express both IAP 12 and alphaVbeta3 2 on their cell surface, we wished to specifically determine whether TS-1 binding to IAP contributes to this enhancement effect.	bind
38105	2	8757	5	13	NULL	NULL	NULL	SMCs	Cell		express					alphaVbeta3	GP				NULL	cell surface	NULL	NULL	NULL	NULL	gw70_circulationres_93_10_925_s_62	14563713	9 Because we have also determined that SMCs express both IAP 12 and alphaVbeta3 2 on their cell surface, we wished to specifically determine whether TS-1 binding to IAP contributes to this enhancement effect.	bind
38106	3	8757	5	13	NULL	NULL	NULL	TS-1	GP		bind					IAP	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_93_10_925_s_62	14563713	9 Because we have also determined that SMCs express both IAP 12 and alphaVbeta3 2 on their cell surface, we wished to specifically determine whether TS-1 binding to IAP contributes to this enhancement effect.	bind
37359	1	8757	7	NULL	NULL	0	NULL	 TS-1 	NULL		bind	NULL				 IAP	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_93_10_925_s_62	14563713	9 Because we have also determined that SMCs express both IAP 12 and alphaVbeta3 2 on their cell surface, we wished to specifically determine whether TS-1 binding to IAP contributes to this enhancement effect.	bind
37360	2	8757	7	NULL	NULL	0	NULL	SMCs	NULL		express	NULL				IAP 12	NULL				NULL	cell surface	0	NULL	NULL	NULL	gw70_circulationres_93_10_925_s_62	14563713	9 Because we have also determined that SMCs express both IAP 12 and alphaVbeta3 2 on their cell surface, we wished to specifically determine whether TS-1 binding to IAP contributes to this enhancement effect.	bind
37361	3	8757	7	NULL	NULL	0	NULL	SMCs	NULL		express	NULL				alphaVbeta3 2	NULL				NULL	cell surface	0	NULL	NULL	NULL	gw70_circulationres_93_10_925_s_62	14563713	9 Because we have also determined that SMCs express both IAP 12 and alphaVbeta3 2 on their cell surface, we wished to specifically determine whether TS-1 binding to IAP contributes to this enhancement effect.	bind
38102	1	8758	5	13	NULL	NULL	NULL	Sp1	GP		bind					Flk-1/KDR	GP			CT-rich recognition sequence within -79 to -68 region of promoter	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_907_s_23	12067897	9 EMSA has demonstrated that expression of human Flk-1/KDR is mediated by Sp1 binding to a CT-rich recognition sequence within the -79 to -68 region of the Flk-1/KDR promoter.	bind
38103	2	8758	5	13	NULL	NULL	NULL	statement 1	Process		mediate					Flk-1/KDR	GP	expression of;;human			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_907_s_23	12067897	9 EMSA has demonstrated that expression of human Flk-1/KDR is mediated by Sp1 binding to a CT-rich recognition sequence within the -79 to -68 region of the Flk-1/KDR promoter.	bind
37362	1	8758	7	NULL	NULL	0	NULL	Sp1	NULL		bind	NULL				Flk-1/KDR	NULL			CT-rich recognition sequence within the -79 to -68 region of  promoter	NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_907_s_23	12067897	9 EMSA has demonstrated that expression of human Flk-1/KDR is mediated by Sp1 binding to a CT-rich recognition sequence within the -79 to -68 region of the Flk-1/KDR promoter.	bind
37363	2	8758	7	10	NULL	0	NULL	statement 1	NULL		mediates	NULL				Flk-1/KDR 	NULL	expression of;; human			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_907_s_23	12067897	9 EMSA has demonstrated that expression of human Flk-1/KDR is mediated by Sp1 binding to a CT-rich recognition sequence within the -79 to -68 region of the Flk-1/KDR promoter.	bind
38099	1	8760	5	13	NULL	NULL	NULL	microbicides	Chemical		interact with					virus	Organism				NULL		NULL	NULL	NULL	NULL	gw70_jantimicrobchemoth_52_6_890_s_67	14613946	9 However, most microbicides intended to interact with the virus bind to the viral envelope glycoproteins (Env).	bind
38100	2	8760	5	13	NULL	NULL	NULL	statement 1	Chemical		bind					Env	GP				NULL		NULL	NULL	NULL	NULL	gw70_jantimicrobchemoth_52_6_890_s_67	14613946	9 However, most microbicides intended to interact with the virus bind to the viral envelope glycoproteins (Env).	bind
38101	3	8760	5	13	NULL	NULL	NULL	Env	GP		is					viral envelope glycoproteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_jantimicrobchemoth_52_6_890_s_67	14613946	9 However, most microbicides intended to interact with the virus bind to the viral envelope glycoproteins (Env).	bind
37365	1	8760	7	NULL	NULL	0	NULL	virus	NULL		binds to	NULL				viral Env	NULL				NULL		0	NULL	NULL	NULL	gw70_jantimicrobchemoth_52_6_890_s_67	14613946	9 However, most microbicides intended to interact with the virus bind to the viral envelope glycoproteins (Env).	bind
37366	2	8760	7	NULL	NULL	0	NULL	microbicides	NULL		interacts with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jantimicrobchemoth_52_6_890_s_67	14613946	9 However, most microbicides intended to interact with the virus bind to the viral envelope glycoproteins (Env).	bind
37367	3	8760	7	NULL	NULL	0	NULL	Env	NULL		is	NULL				envelope glycoproteins	NULL				NULL		0	NULL	NULL	NULL	gw70_jantimicrobchemoth_52_6_890_s_67	14613946	9 However, most microbicides intended to interact with the virus bind to the viral envelope glycoproteins (Env).	bind
38115	1	8761	5	13	NULL	NULL	NULL	MCP-1	GP		bind					CCR2 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_969_s_155	12067906	9 However, this drug inhibits neither the activity of MCP-1 nor the binding of MCP-1 to its receptor CCR2.	bind
37368	1	8761	7	NULL	NULL	0	NULL	 MCP-1	NULL		binds to	NULL				CCR2 receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_969_s_155	12067906	9 However, this drug inhibits neither the activity of MCP-1 nor the binding of MCP-1 to its receptor CCR2.	bind
38117	1	8762	5	13	NULL	NULL	NULL	Sp1	GP		bind					PON1	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_11_2083_s_169	14500290	9 In recent studies, we have demonstrated that the polymorphism modulates binding of Sp1 to the  PON1 promoter.	bind
38118	2	8762	5	13	NULL	NULL	NULL	polymorphism	Process		modulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_11_2083_s_169	14500290	9 In recent studies, we have demonstrated that the polymorphism modulates binding of Sp1 to the  PON1 promoter.	bind
37369	1	8762	7	NULL	NULL	0	NULL	Sp1 	NULL		bind	NULL				PON1	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_11_2083_s_169	14500290	9 In recent studies, we have demonstrated that the polymorphism modulates binding of Sp1 to the  PON1 promoter.	bind
37370	2	8762	7	NULL	NULL	0	NULL	polymorphism	NULL		modulates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_11_2083_s_169	14500290	9 In recent studies, we have demonstrated that the polymorphism modulates binding of Sp1 to the  PON1 promoter.	bind
38712	1	8763	5	13	NULL	NULL	NULL	c-fos	GP		respond to					Ca2+	Chemical				NULL	neurons	NULL	NULL	NULL	NULL	gw70_circulationres_95_4_406_s_177	15256479	9 Interestingly, the c-fos response to Ca2+ in neurons is partially regulated by SRF phosphorylation by CaMK and increased SRF binding to the c-fos CArG. 25 Therefore, it is plausible that VGCC activation stimulates multiple distinct signaling pathways in SMCs that regulate distinct subsets of genes, such as genes that define the "`contractile"' SMC, eg, SM alpha-actin and SMMHC, versus genes involved in mediating cell growth, eg, c-fos.	bind
38713	2	8763	5	13	NULL	NULL	NULL	SRF	GP		is phosphorylated by					CaMK	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_4_406_s_177	15256479	9 Interestingly, the c-fos response to Ca2+ in neurons is partially regulated by SRF phosphorylation by CaMK and increased SRF binding to the c-fos CArG. 25 Therefore, it is plausible that VGCC activation stimulates multiple distinct signaling pathways in SMCs that regulate distinct subsets of genes, such as genes that define the "`contractile"' SMC, eg, SM alpha-actin and SMMHC, versus genes involved in mediating cell growth, eg, c-fos.	bind
38714	3	8763	5	13	NULL	NULL	NULL	statement 2	Process		regulates		partially			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_4_406_s_177	15256479	9 Interestingly, the c-fos response to Ca2+ in neurons is partially regulated by SRF phosphorylation by CaMK and increased SRF binding to the c-fos CArG. 25 Therefore, it is plausible that VGCC activation stimulates multiple distinct signaling pathways in SMCs that regulate distinct subsets of genes, such as genes that define the "`contractile"' SMC, eg, SM alpha-actin and SMMHC, versus genes involved in mediating cell growth, eg, c-fos.	bind
38715	4	8763	5	13	NULL	NULL	NULL	SRF	GP		bind					c-fos	GP			CArG	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_4_406_s_177	15256479	9 Interestingly, the c-fos response to Ca2+ in neurons is partially regulated by SRF phosphorylation by CaMK and increased SRF binding to the c-fos CArG. 25 Therefore, it is plausible that VGCC activation stimulates multiple distinct signaling pathways in SMCs that regulate distinct subsets of genes, such as genes that define the "`contractile"' SMC, eg, SM alpha-actin and SMMHC, versus genes involved in mediating cell growth, eg, c-fos.	bind
38716	5	8763	5	13	NULL	NULL	NULL	statement 4	Process	increased	regulates		partially			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_4_406_s_177	15256479	9 Interestingly, the c-fos response to Ca2+ in neurons is partially regulated by SRF phosphorylation by CaMK and increased SRF binding to the c-fos CArG. 25 Therefore, it is plausible that VGCC activation stimulates multiple distinct signaling pathways in SMCs that regulate distinct subsets of genes, such as genes that define the "`contractile"' SMC, eg, SM alpha-actin and SMMHC, versus genes involved in mediating cell growth, eg, c-fos.	bind
38717	6	8763	5	13	NULL	NULL	NULL	VGCC	GP	activation of	stimulate					signaling pathways	Process	multiple distinct			NULL	SMCs	NULL	NULL	NULL	NULL	gw70_circulationres_95_4_406_s_177	15256479	9 Interestingly, the c-fos response to Ca2+ in neurons is partially regulated by SRF phosphorylation by CaMK and increased SRF binding to the c-fos CArG. 25 Therefore, it is plausible that VGCC activation stimulates multiple distinct signaling pathways in SMCs that regulate distinct subsets of genes, such as genes that define the "`contractile"' SMC, eg, SM alpha-actin and SMMHC, versus genes involved in mediating cell growth, eg, c-fos.	bind
38718	7	8763	5	13	NULL	NULL	NULL	statement 6	Process		regulates					SM alpha-actin gene	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_4_406_s_177	15256479	9 Interestingly, the c-fos response to Ca2+ in neurons is partially regulated by SRF phosphorylation by CaMK and increased SRF binding to the c-fos CArG. 25 Therefore, it is plausible that VGCC activation stimulates multiple distinct signaling pathways in SMCs that regulate distinct subsets of genes, such as genes that define the "`contractile"' SMC, eg, SM alpha-actin and SMMHC, versus genes involved in mediating cell growth, eg, c-fos.	bind
38719	8	8763	5	13	NULL	NULL	NULL	statement 6	Process		regulates					SMMHC gene	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_4_406_s_177	15256479	9 Interestingly, the c-fos response to Ca2+ in neurons is partially regulated by SRF phosphorylation by CaMK and increased SRF binding to the c-fos CArG. 25 Therefore, it is plausible that VGCC activation stimulates multiple distinct signaling pathways in SMCs that regulate distinct subsets of genes, such as genes that define the "`contractile"' SMC, eg, SM alpha-actin and SMMHC, versus genes involved in mediating cell growth, eg, c-fos.	bind
38720	9	8763	5	13	NULL	NULL	NULL	statement 6	Process		regulates					c-fos gene	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_4_406_s_177	15256479	9 Interestingly, the c-fos response to Ca2+ in neurons is partially regulated by SRF phosphorylation by CaMK and increased SRF binding to the c-fos CArG. 25 Therefore, it is plausible that VGCC activation stimulates multiple distinct signaling pathways in SMCs that regulate distinct subsets of genes, such as genes that define the "`contractile"' SMC, eg, SM alpha-actin and SMMHC, versus genes involved in mediating cell growth, eg, c-fos.	bind
38721	10	8763	5	13	NULL	NULL	NULL	c-fos gene	GP		mediate					cell growth	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_4_406_s_177	15256479	9 Interestingly, the c-fos response to Ca2+ in neurons is partially regulated by SRF phosphorylation by CaMK and increased SRF binding to the c-fos CArG. 25 Therefore, it is plausible that VGCC activation stimulates multiple distinct signaling pathways in SMCs that regulate distinct subsets of genes, such as genes that define the "`contractile"' SMC, eg, SM alpha-actin and SMMHC, versus genes involved in mediating cell growth, eg, c-fos.	bind
38722	11	8763	5	13	NULL	NULL	NULL	SM alpha-actin gene	GP		defines					"`contractile"' SMC	Cell				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_4_406_s_177	15256479	9 Interestingly, the c-fos response to Ca2+ in neurons is partially regulated by SRF phosphorylation by CaMK and increased SRF binding to the c-fos CArG. 25 Therefore, it is plausible that VGCC activation stimulates multiple distinct signaling pathways in SMCs that regulate distinct subsets of genes, such as genes that define the "`contractile"' SMC, eg, SM alpha-actin and SMMHC, versus genes involved in mediating cell growth, eg, c-fos.	bind
38723	12	8763	5	13	NULL	NULL	NULL	SMMHC gene	GP		defines					"`contractile"' SMC	Cell				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_4_406_s_177	15256479	9 Interestingly, the c-fos response to Ca2+ in neurons is partially regulated by SRF phosphorylation by CaMK and increased SRF binding to the c-fos CArG. 25 Therefore, it is plausible that VGCC activation stimulates multiple distinct signaling pathways in SMCs that regulate distinct subsets of genes, such as genes that define the "`contractile"' SMC, eg, SM alpha-actin and SMMHC, versus genes involved in mediating cell growth, eg, c-fos.	bind
37373	1	8763	7	NULL	NULL	0	NULL	 c-fos	NULL		respond to	NULL				Ca2+	NULL				NULL	neurons	0	NULL	NULL	NULL	gw70_circulationres_95_4_406_s_177	15256479	9 Interestingly, the c-fos response to Ca2+ in neurons is partially regulated by SRF phosphorylation by CaMK and increased SRF binding to the c-fos CArG. 25 Therefore, it is plausible that VGCC activation stimulates multiple distinct signaling pathways in SMCs that regulate distinct subsets of genes, such as genes that define the "`contractile"' SMC, eg, SM alpha-actin and SMMHC, versus genes involved in mediating cell growth, eg, c-fos.	bind
37374	2	8763	7	NULL	NULL	0	NULL	CaMK	NULL		phosphorylates	NULL				SRF	NULL				NULL	neurons	NULL	NULL	NULL	NULL	gw70_circulationres_95_4_406_s_177	15256479	9 Interestingly, the c-fos response to Ca2+ in neurons is partially regulated by SRF phosphorylation by CaMK and increased SRF binding to the c-fos CArG. 25 Therefore, it is plausible that VGCC activation stimulates multiple distinct signaling pathways in SMCs that regulate distinct subsets of genes, such as genes that define the "`contractile"' SMC, eg, SM alpha-actin and SMMHC, versus genes involved in mediating cell growth, eg, c-fos.	bind
37376	3	8763	7	NULL	NULL	0	NULL	statement 2	NULL		regulates	NULL	partially			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_4_406_s_177	15256479	9 Interestingly, the c-fos response to Ca2+ in neurons is partially regulated by SRF phosphorylation by CaMK and increased SRF binding to the c-fos CArG. 25 Therefore, it is plausible that VGCC activation stimulates multiple distinct signaling pathways in SMCs that regulate distinct subsets of genes, such as genes that define the "`contractile"' SMC, eg, SM alpha-actin and SMMHC, versus genes involved in mediating cell growth, eg, c-fos.	bind
37378	4	8763	7	NULL	NULL	0	NULL	SRF	NULL		bind	NULL				c-fos	NULL			CArG	NULL		0	NULL	NULL	NULL	gw70_circulationres_95_4_406_s_177	15256479	9 Interestingly, the c-fos response to Ca2+ in neurons is partially regulated by SRF phosphorylation by CaMK and increased SRF binding to the c-fos CArG. 25 Therefore, it is plausible that VGCC activation stimulates multiple distinct signaling pathways in SMCs that regulate distinct subsets of genes, such as genes that define the "`contractile"' SMC, eg, SM alpha-actin and SMMHC, versus genes involved in mediating cell growth, eg, c-fos.	bind
37380	5	8763	7	NULL	NULL	0	NULL	statement 4	NULL	increase of	regulates	NULL	partially			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_4_406_s_177	15256479	9 Interestingly, the c-fos response to Ca2+ in neurons is partially regulated by SRF phosphorylation by CaMK and increased SRF binding to the c-fos CArG. 25 Therefore, it is plausible that VGCC activation stimulates multiple distinct signaling pathways in SMCs that regulate distinct subsets of genes, such as genes that define the "`contractile"' SMC, eg, SM alpha-actin and SMMHC, versus genes involved in mediating cell growth, eg, c-fos.	bind
37384	6	8763	7	NULL	NULL	0	NULL	VGCC	NULL	activation of	stimulates	NULL				multiple distinct signaling pathways	NULL				NULL	SMCs	0	NULL	NULL	NULL	gw70_circulationres_95_4_406_s_177	15256479	9 Interestingly, the c-fos response to Ca2+ in neurons is partially regulated by SRF phosphorylation by CaMK and increased SRF binding to the c-fos CArG. 25 Therefore, it is plausible that VGCC activation stimulates multiple distinct signaling pathways in SMCs that regulate distinct subsets of genes, such as genes that define the "`contractile"' SMC, eg, SM alpha-actin and SMMHC, versus genes involved in mediating cell growth, eg, c-fos.	bind
37385	7	8763	7	NULL	NULL	0	NULL	statement 6	NULL		regulate	NULL				SM alpha-actin	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_95_4_406_s_177	15256479	9 Interestingly, the c-fos response to Ca2+ in neurons is partially regulated by SRF phosphorylation by CaMK and increased SRF binding to the c-fos CArG. 25 Therefore, it is plausible that VGCC activation stimulates multiple distinct signaling pathways in SMCs that regulate distinct subsets of genes, such as genes that define the "`contractile"' SMC, eg, SM alpha-actin and SMMHC, versus genes involved in mediating cell growth, eg, c-fos.	bind
37386	8	8763	7	NULL	NULL	0	NULL	SM alpha-actin	NULL		define	NULL				contractile SMC	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_95_4_406_s_177	15256479	9 Interestingly, the c-fos response to Ca2+ in neurons is partially regulated by SRF phosphorylation by CaMK and increased SRF binding to the c-fos CArG. 25 Therefore, it is plausible that VGCC activation stimulates multiple distinct signaling pathways in SMCs that regulate distinct subsets of genes, such as genes that define the "`contractile"' SMC, eg, SM alpha-actin and SMMHC, versus genes involved in mediating cell growth, eg, c-fos.	bind
37387	9	8763	7	NULL	NULL	0	NULL	statement 6	NULL		regulate	NULL				SMMHC	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_95_4_406_s_177	15256479	9 Interestingly, the c-fos response to Ca2+ in neurons is partially regulated by SRF phosphorylation by CaMK and increased SRF binding to the c-fos CArG. 25 Therefore, it is plausible that VGCC activation stimulates multiple distinct signaling pathways in SMCs that regulate distinct subsets of genes, such as genes that define the "`contractile"' SMC, eg, SM alpha-actin and SMMHC, versus genes involved in mediating cell growth, eg, c-fos.	bind
37390	10	8763	7	NULL	NULL	0	NULL	SMMHC	NULL		define	NULL				contractile SMC	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_95_4_406_s_177	15256479	9 Interestingly, the c-fos response to Ca2+ in neurons is partially regulated by SRF phosphorylation by CaMK and increased SRF binding to the c-fos CArG. 25 Therefore, it is plausible that VGCC activation stimulates multiple distinct signaling pathways in SMCs that regulate distinct subsets of genes, such as genes that define the "`contractile"' SMC, eg, SM alpha-actin and SMMHC, versus genes involved in mediating cell growth, eg, c-fos.	bind
37392	11	8763	7	10	NULL	0	NULL	c-fos	NULL		mediates	NULL				cell growth	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_4_406_s_177	15256479	9 Interestingly, the c-fos response to Ca2+ in neurons is partially regulated by SRF phosphorylation by CaMK and increased SRF binding to the c-fos CArG. 25 Therefore, it is plausible that VGCC activation stimulates multiple distinct signaling pathways in SMCs that regulate distinct subsets of genes, such as genes that define the "`contractile"' SMC, eg, SM alpha-actin and SMMHC, versus genes involved in mediating cell growth, eg, c-fos.	bind
37395	12	8763	7	NULL	NULL	0	NULL	statement 6	NULL		regulate	NULL				statement 11	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_95_4_406_s_177	15256479	9 Interestingly, the c-fos response to Ca2+ in neurons is partially regulated by SRF phosphorylation by CaMK and increased SRF binding to the c-fos CArG. 25 Therefore, it is plausible that VGCC activation stimulates multiple distinct signaling pathways in SMCs that regulate distinct subsets of genes, such as genes that define the "`contractile"' SMC, eg, SM alpha-actin and SMMHC, versus genes involved in mediating cell growth, eg, c-fos.	bind
38119	1	8764	5	13	NULL	NULL	NULL	RI	GP		associate with								RI-subunits		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_8_993_s_32	16645149	9 RI associates with other RI-subunits, whereas RII binds only other RII-subunits.	bind
38120	2	8764	5	13	NULL	NULL	NULL	RII	GP		bind		only						RII-subunits		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_8_993_s_32	16645149	9 RI associates with other RI-subunits, whereas RII binds only other RII-subunits.	bind
37397	1	8764	7	10	NULL	0	NULL	RI	NULL		associate with	NULL					NULL		RI-subunits		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_8_993_s_32	16645149	9 RI associates with other RI-subunits, whereas RII binds only other RII-subunits.	bind
37398	2	8764	7	10	NULL	0	NULL	RII	NULL		binds	NULL	only				NULL		RII-subunit		NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_8_993_s_32	16645149	9 RI associates with other RI-subunits, whereas RII binds only other RII-subunits.	bind
38121	1	8765	5	13	NULL	NULL	NULL	FXa	GP		bind					TF FVIIa	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2964_s_21	9409283	9 Then TFPI uses the tandem Kunitz-type domains in its structure to form a quaternary complex with FXa bound to TF FVIIa.	bind
38122	2	8765	5	13	NULL	NULL	NULL	TFPI	GP		bind			tandem Kunitz-type domains		statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2964_s_21	9409283	9 Then TFPI uses the tandem Kunitz-type domains in its structure to form a quaternary complex with FXa bound to TF FVIIa.	bind
38123	3	8765	5	13	NULL	NULL	NULL	statement 2	GP		forms					quaternary complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2964_s_21	9409283	9 Then TFPI uses the tandem Kunitz-type domains in its structure to form a quaternary complex with FXa bound to TF FVIIa.	bind
37399	1	8765	7	NULL	NULL	0	NULL	FXa	NULL		bind	NULL				TF FVIIa	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2964_s_21	9409283	9 Then TFPI uses the tandem Kunitz-type domains in its structure to form a quaternary complex with FXa bound to TF FVIIa.	bind
37400	2	8765	7	10	NULL	0	NULL	TFPI	NULL		bind	NULL		tandem Kunitz-type domains		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2964_s_21	9409283	9 Then TFPI uses the tandem Kunitz-type domains in its structure to form a quaternary complex with FXa bound to TF FVIIa.	bind
46757	3	8765	7	10	NULL	0	NULL	statement 2	NULL		forms	NULL				quaternary complex	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2964_s_21	9409283	9 Then TFPI uses the tandem Kunitz-type domains in its structure to form a quaternary complex with FXa bound to TF FVIIa.	bind
38124	1	8766	5	13	NULL	NULL	NULL	yeasts	Organism		bind					BSA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jantimicrobchemoth_43_4_583_s_90	10350392	9 These agents do not significantly affect the binding of yeasts to BSA.	bind
37401	1	8766	7	NULL	NULL	0	NULL	 yeasts 	NULL		bind	NULL				BSA	NULL				NULL		0	NULL	NULL	NULL	gw60_jantimicrobchemoth_43_4_583_s_90	10350392	9 These agents do not significantly affect the binding of yeasts to BSA.	bind
38125	1	8767	5	13	NULL	NULL	NULL	Smad3	GP		bind					SM22alpha	GP			SBE region of promoter	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_circulationres_97_10_983_s_80	16224064	9 To determine whether Smad3 binds to the SBE region of the SM22alpha promoter in vivo, we performed ChIP assays on cultured cells.	bind
37412	1	8767	7	NULL	NULL	0	NULL	 Smad3	NULL		binds to	NULL				SM22alpha	NULL			SBE region of promoter	NULL	in vivo	0	NULL	NULL	NULL	gw70_circulationres_97_10_983_s_80	16224064	9 To determine whether Smad3 binds to the SBE region of the SM22alpha promoter in vivo, we performed ChIP assays on cultured cells.	bind
38126	1	8768	5	13	NULL	NULL	NULL	VEGF-B	GP		bind					VEGFR-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_5_664_s_31	14739162	9 VEGF-B and PlGF bind to VEGFR-1 and modulate the effects of VEGF-A, but their roles in stimulation of angiogenesis remain controversial.	bind
38127	2	8768	5	13	NULL	NULL	NULL	statement 1	Process		modulates					VEGF-A	GP	effects of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_5_664_s_31	14739162	9 VEGF-B and PlGF bind to VEGFR-1 and modulate the effects of VEGF-A, but their roles in stimulation of angiogenesis remain controversial.	bind
38128	3	8768	5	13	NULL	NULL	NULL	PlGF	GP		bind					VEGFR-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_94_5_664_s_31	14739162	9 VEGF-B and PlGF bind to VEGFR-1 and modulate the effects of VEGF-A, but their roles in stimulation of angiogenesis remain controversial.	bind
38129	4	8768	5	NULL	NULL	0	NULL	statement 3	NULL		modulates	NULL				VEGF-A	NULL	effects of			NULL		0	NULL	NULL	NULL	gw70_circulationres_94_5_664_s_31	14739162	9 VEGF-B and PlGF bind to VEGFR-1 and modulate the effects of VEGF-A, but their roles in stimulation of angiogenesis remain controversial.	bind
37413	1	8768	7	NULL	NULL	0	NULL	VEGF-B 	NULL		bind	NULL				VEGFR-1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_5_664_s_31	14739162	9 VEGF-B and PlGF bind to VEGFR-1 and modulate the effects of VEGF-A, but their roles in stimulation of angiogenesis remain controversial.	bind
37414	2	8768	7	NULL	NULL	0	NULL	PlGF	NULL		bind	NULL				VEGFR-1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_94_5_664_s_31	14739162	9 VEGF-B and PlGF bind to VEGFR-1 and modulate the effects of VEGF-A, but their roles in stimulation of angiogenesis remain controversial.	bind
37415	3	8768	7	NULL	NULL	0	NULL	statement 1	NULL		modulate	NULL				VEGF-A	NULL	effects of			NULL		0	NULL	NULL	NULL	gw70_circulationres_94_5_664_s_31	14739162	9 VEGF-B and PlGF bind to VEGFR-1 and modulate the effects of VEGF-A, but their roles in stimulation of angiogenesis remain controversial.	bind
37416	4	8768	7	NULL	NULL	0	NULL	statement 2	NULL		modulate	NULL				VEGF-A	NULL	effects of			NULL		0	NULL	NULL	NULL	gw70_circulationres_94_5_664_s_31	14739162	9 VEGF-B and PlGF bind to VEGFR-1 and modulate the effects of VEGF-A, but their roles in stimulation of angiogenesis remain controversial.	bind
38256	1	8769	5	13	NULL	NULL	NULL	Cdc37	GP		bind		potentially			eNOS	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_335_s_204	16410463	9 With this in mind, we hypothesize that Cdc37 bound to the eNOS in the absence of other regulatory proteins serves a protective function inhibiting uncoupled or unregulated eNOS activity and that overexpression of Cdc37 interferes with the proper interactions of eNOS with Hsp90 and Akt and subsequent activation.	bind
38257	2	8769	5	13	NULL	NULL	NULL	statement 1	Process		in the absence of		potentially			regulatory proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_335_s_204	16410463	9 With this in mind, we hypothesize that Cdc37 bound to the eNOS in the absence of other regulatory proteins serves a protective function inhibiting uncoupled or unregulated eNOS activity and that overexpression of Cdc37 interferes with the proper interactions of eNOS with Hsp90 and Akt and subsequent activation.	bind
38258	3	8769	5	13	NULL	NULL	NULL	statement 2	Process		serves		potentially			protective function	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_335_s_204	16410463	9 With this in mind, we hypothesize that Cdc37 bound to the eNOS in the absence of other regulatory proteins serves a protective function inhibiting uncoupled or unregulated eNOS activity and that overexpression of Cdc37 interferes with the proper interactions of eNOS with Hsp90 and Akt and subsequent activation.	bind
38259	4	8769	5	13	NULL	NULL	NULL	statement 3	Process		inhibit		potentially			eNOS	GP	uncoupled;;activity of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_335_s_204	16410463	9 With this in mind, we hypothesize that Cdc37 bound to the eNOS in the absence of other regulatory proteins serves a protective function inhibiting uncoupled or unregulated eNOS activity and that overexpression of Cdc37 interferes with the proper interactions of eNOS with Hsp90 and Akt and subsequent activation.	bind
38260	5	8769	5	13	NULL	NULL	NULL	statement 3	Process		inhibit		potentially			eNOS	GP	unregulated;;activity of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_335_s_204	16410463	9 With this in mind, we hypothesize that Cdc37 bound to the eNOS in the absence of other regulatory proteins serves a protective function inhibiting uncoupled or unregulated eNOS activity and that overexpression of Cdc37 interferes with the proper interactions of eNOS with Hsp90 and Akt and subsequent activation.	bind
38261	6	8769	5	13	NULL	NULL	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_335_s_204	16410463	9 With this in mind, we hypothesize that Cdc37 bound to the eNOS in the absence of other regulatory proteins serves a protective function inhibiting uncoupled or unregulated eNOS activity and that overexpression of Cdc37 interferes with the proper interactions of eNOS with Hsp90 and Akt and subsequent activation.	bind
38262	7	8769	5	13	NULL	NULL	NULL	eNOS	GP		interact with					Hsp90 	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_335_s_204	16410463	9 With this in mind, we hypothesize that Cdc37 bound to the eNOS in the absence of other regulatory proteins serves a protective function inhibiting uncoupled or unregulated eNOS activity and that overexpression of Cdc37 interferes with the proper interactions of eNOS with Hsp90 and Akt and subsequent activation.	bind
38263	8	8769	5	13	NULL	NULL	NULL	eNOS	GP		interact with					Akt	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_335_s_204	16410463	9 With this in mind, we hypothesize that Cdc37 bound to the eNOS in the absence of other regulatory proteins serves a protective function inhibiting uncoupled or unregulated eNOS activity and that overexpression of Cdc37 interferes with the proper interactions of eNOS with Hsp90 and Akt and subsequent activation.	bind
38264	9	8769	5	13	NULL	NULL	NULL	statement 7	Process		activates		subsequently			Hsp90	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_335_s_204	16410463	9 With this in mind, we hypothesize that Cdc37 bound to the eNOS in the absence of other regulatory proteins serves a protective function inhibiting uncoupled or unregulated eNOS activity and that overexpression of Cdc37 interferes with the proper interactions of eNOS with Hsp90 and Akt and subsequent activation.	bind
38265	10	8769	5	13	NULL	NULL	NULL	statement 8	Process		activates		subsequently			Akt	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_335_s_204	16410463	9 With this in mind, we hypothesize that Cdc37 bound to the eNOS in the absence of other regulatory proteins serves a protective function inhibiting uncoupled or unregulated eNOS activity and that overexpression of Cdc37 interferes with the proper interactions of eNOS with Hsp90 and Akt and subsequent activation.	bind
38266	11	8769	5	13	NULL	NULL	NULL	Cdc37	GP	overexpression of	interfere with		potentially			statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_335_s_204	16410463	9 With this in mind, we hypothesize that Cdc37 bound to the eNOS in the absence of other regulatory proteins serves a protective function inhibiting uncoupled or unregulated eNOS activity and that overexpression of Cdc37 interferes with the proper interactions of eNOS with Hsp90 and Akt and subsequent activation.	bind
38267	12	8769	5	13	NULL	NULL	NULL	Cdc37	GP	overexpression of	interfere with		potentially			statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_335_s_204	16410463	9 With this in mind, we hypothesize that Cdc37 bound to the eNOS in the absence of other regulatory proteins serves a protective function inhibiting uncoupled or unregulated eNOS activity and that overexpression of Cdc37 interferes with the proper interactions of eNOS with Hsp90 and Akt and subsequent activation.	bind
38268	13	8769	5	13	NULL	NULL	NULL	Cdc37	GP	overexpression of	interfere with		potentially			statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_335_s_204	16410463	9 With this in mind, we hypothesize that Cdc37 bound to the eNOS in the absence of other regulatory proteins serves a protective function inhibiting uncoupled or unregulated eNOS activity and that overexpression of Cdc37 interferes with the proper interactions of eNOS with Hsp90 and Akt and subsequent activation.	bind
38269	14	8769	5	13	NULL	NULL	NULL	Cdc37	GP	overexpression of	interfere with		potentially			statement 10	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_335_s_204	16410463	9 With this in mind, we hypothesize that Cdc37 bound to the eNOS in the absence of other regulatory proteins serves a protective function inhibiting uncoupled or unregulated eNOS activity and that overexpression of Cdc37 interferes with the proper interactions of eNOS with Hsp90 and Akt and subsequent activation.	bind
37419	1	8769	7	NULL	NULL	0	NULL	Cdc37 	NULL		bind	NULL				eNOS	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_3_335_s_204	16410463	9 With this in mind, we hypothesize that Cdc37 bound to the eNOS in the absence of other regulatory proteins serves a protective function inhibiting uncoupled or unregulated eNOS activity and that overexpression of Cdc37 interferes with the proper interactions of eNOS with Hsp90 and Akt and subsequent activation.	bind
37420	2	8769	7	NULL	NULL	0	NULL	statement 1	NULL		in the absence of	NULL				regulatory proteins	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_3_335_s_204	16410463	9 With this in mind, we hypothesize that Cdc37 bound to the eNOS in the absence of other regulatory proteins serves a protective function inhibiting uncoupled or unregulated eNOS activity and that overexpression of Cdc37 interferes with the proper interactions of eNOS with Hsp90 and Akt and subsequent activation.	bind
37422	3	8769	7	10	NULL	0	NULL	statement 2	NULL		inhibit	NULL				eNOS	NULL	uncoupled;; activity of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_335_s_204	16410463	9 With this in mind, we hypothesize that Cdc37 bound to the eNOS in the absence of other regulatory proteins serves a protective function inhibiting uncoupled or unregulated eNOS activity and that overexpression of Cdc37 interferes with the proper interactions of eNOS with Hsp90 and Akt and subsequent activation.	bind
37423	4	8769	7	10	NULL	0	NULL	statement 2	NULL		inhibit	NULL				eNOS	NULL	unregulated;; activity of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_3_335_s_204	16410463	9 With this in mind, we hypothesize that Cdc37 bound to the eNOS in the absence of other regulatory proteins serves a protective function inhibiting uncoupled or unregulated eNOS activity and that overexpression of Cdc37 interferes with the proper interactions of eNOS with Hsp90 and Akt and subsequent activation.	bind
37435	5	8769	7	NULL	NULL	0	NULL	statement 2	NULL		serves a	NULL				protective funtion	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_3_335_s_204	16410463	9 With this in mind, we hypothesize that Cdc37 bound to the eNOS in the absence of other regulatory proteins serves a protective function inhibiting uncoupled or unregulated eNOS activity and that overexpression of Cdc37 interferes with the proper interactions of eNOS with Hsp90 and Akt and subsequent activation.	bind
37436	6	8769	7	NULL	NULL	0	NULL	statement 5	NULL		occurs by	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_3_335_s_204	16410463	9 With this in mind, we hypothesize that Cdc37 bound to the eNOS in the absence of other regulatory proteins serves a protective function inhibiting uncoupled or unregulated eNOS activity and that overexpression of Cdc37 interferes with the proper interactions of eNOS with Hsp90 and Akt and subsequent activation.	bind
37437	7	8769	7	NULL	NULL	0	NULL	statement 5	NULL		occurs by	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_3_335_s_204	16410463	9 With this in mind, we hypothesize that Cdc37 bound to the eNOS in the absence of other regulatory proteins serves a protective function inhibiting uncoupled or unregulated eNOS activity and that overexpression of Cdc37 interferes with the proper interactions of eNOS with Hsp90 and Akt and subsequent activation.	bind
37438	8	8769	7	NULL	NULL	0	NULL	eNOS	NULL		interacts with	NULL				Hsp90	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_3_335_s_204	16410463	9 With this in mind, we hypothesize that Cdc37 bound to the eNOS in the absence of other regulatory proteins serves a protective function inhibiting uncoupled or unregulated eNOS activity and that overexpression of Cdc37 interferes with the proper interactions of eNOS with Hsp90 and Akt and subsequent activation.	bind
37439	9	8769	7	NULL	NULL	0	NULL	eNOS	NULL		interacts with	NULL				Akt	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_3_335_s_204	16410463	9 With this in mind, we hypothesize that Cdc37 bound to the eNOS in the absence of other regulatory proteins serves a protective function inhibiting uncoupled or unregulated eNOS activity and that overexpression of Cdc37 interferes with the proper interactions of eNOS with Hsp90 and Akt and subsequent activation.	bind
37440	10	8769	7	NULL	NULL	0	NULL	Cdc37	NULL	overexpression of	interferes with	NULL				statement 8	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_3_335_s_204	16410463	9 With this in mind, we hypothesize that Cdc37 bound to the eNOS in the absence of other regulatory proteins serves a protective function inhibiting uncoupled or unregulated eNOS activity and that overexpression of Cdc37 interferes with the proper interactions of eNOS with Hsp90 and Akt and subsequent activation.	bind
37441	11	8769	7	NULL	NULL	0	NULL	Cdc37	NULL	overexpression of	interferes with	NULL				statement 9	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_3_335_s_204	16410463	9 With this in mind, we hypothesize that Cdc37 bound to the eNOS in the absence of other regulatory proteins serves a protective function inhibiting uncoupled or unregulated eNOS activity and that overexpression of Cdc37 interferes with the proper interactions of eNOS with Hsp90 and Akt and subsequent activation.	bind
38270	1	8770	5	13	NULL	NULL	NULL	67LR	GP		bind					laminin beta1	GP		cysteine-rich domain of short arm of		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_307_s_15	11786424	9, 10  his receptor (designated 67LR) binds to a cysteine-rich domain of the short arm of laminin beta1.	bind
56426	2	8770	5	13	NULL	NULL	NULL	67LR	GP		is 					his receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_307_s_15	11786424	9, 10  his receptor (designated 67LR) binds to a cysteine-rich domain of the short arm of laminin beta1.	bind
37442	1	8770	7	NULL	NULL	0	NULL	his receptor	NULL		binds to	NULL				laminin beta1	NULL		cysteine-rich domain of the short arm of 		NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_1_307_s_15	11786424	9, 10  his receptor (designated 67LR) binds to a cysteine-rich domain of the short arm of laminin beta1.	bind
37443	2	8770	7	NULL	NULL	0	NULL	his receptor	NULL		is	NULL				67LR	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_1_307_s_15	11786424	9, 10  his receptor (designated 67LR) binds to a cysteine-rich domain of the short arm of laminin beta1.	bind
38271	1	8771	5	13	NULL	NULL	NULL	Ang-1	GP		bind					Tie-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_773_s_13	11891175	9, 13- 15  Ang-1 binds and induces autophosphorylation of Tie-2, 10  promoting endothelial cell migration, 16  sprouting, 17, 18  and survival 19, 20  in vitro; and increases new vessel growth, branching, maturation, and integrity  in vivo.	bind
38272	2	8771	5	13	NULL	NULL	NULL	statement 1	Process		induce					Tie-2	GP	autophosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_773_s_13	11891175	9, 13- 15  Ang-1 binds and induces autophosphorylation of Tie-2, 10  promoting endothelial cell migration, 16  sprouting, 17, 18  and survival 19, 20  in vitro; and increases new vessel growth, branching, maturation, and integrity  in vivo.	bind
38273	3	8771	5	13	NULL	NULL	NULL	statement 2	Process		promotes					endothelial cell	Cell	migration of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_773_s_13	11891175	9, 13- 15  Ang-1 binds and induces autophosphorylation of Tie-2, 10  promoting endothelial cell migration, 16  sprouting, 17, 18  and survival 19, 20  in vitro; and increases new vessel growth, branching, maturation, and integrity  in vivo.	bind
38275	4	8771	5	13	NULL	NULL	NULL	statement 2	Process		promotes					endothelial cell	Cell	sprouting of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_773_s_13	11891175	9, 13- 15  Ang-1 binds and induces autophosphorylation of Tie-2, 10  promoting endothelial cell migration, 16  sprouting, 17, 18  and survival 19, 20  in vitro; and increases new vessel growth, branching, maturation, and integrity  in vivo.	bind
38276	5	8771	5	13	NULL	NULL	NULL	statement 2	Process		promotes					endothelial cell	Cell	survival of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_773_s_13	11891175	9, 13- 15  Ang-1 binds and induces autophosphorylation of Tie-2, 10  promoting endothelial cell migration, 16  sprouting, 17, 18  and survival 19, 20  in vitro; and increases new vessel growth, branching, maturation, and integrity  in vivo.	bind
38283	6	8771	5	13	NULL	NULL	NULL	statement 2	Process		increase					new vessel	OrganismPart	growth of			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_773_s_13	11891175	9, 13- 15  Ang-1 binds and induces autophosphorylation of Tie-2, 10  promoting endothelial cell migration, 16  sprouting, 17, 18  and survival 19, 20  in vitro; and increases new vessel growth, branching, maturation, and integrity  in vivo.	bind
38284	7	8771	5	13	NULL	NULL	NULL	statement 2	Process		increase					new vessel	OrganismPart	branching of			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_773_s_13	11891175	9, 13- 15  Ang-1 binds and induces autophosphorylation of Tie-2, 10  promoting endothelial cell migration, 16  sprouting, 17, 18  and survival 19, 20  in vitro; and increases new vessel growth, branching, maturation, and integrity  in vivo.	bind
38285	8	8771	5	13	NULL	NULL	NULL	statement 2	Process		increase					new vessel	OrganismPart	maturation of			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_773_s_13	11891175	9, 13- 15  Ang-1 binds and induces autophosphorylation of Tie-2, 10  promoting endothelial cell migration, 16  sprouting, 17, 18  and survival 19, 20  in vitro; and increases new vessel growth, branching, maturation, and integrity  in vivo.	bind
38286	9	8771	5	13	NULL	NULL	NULL	statement 2	Process		increase					new vessel	OrganismPart	integrity of			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_773_s_13	11891175	9, 13- 15  Ang-1 binds and induces autophosphorylation of Tie-2, 10  promoting endothelial cell migration, 16  sprouting, 17, 18  and survival 19, 20  in vitro; and increases new vessel growth, branching, maturation, and integrity  in vivo.	bind
37444	1	8771	7	NULL	NULL	0	NULL	Ang-1	NULL		binds	NULL				Tie-2	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_3_773_s_13	11891175	9, 13- 15  Ang-1 binds and induces autophosphorylation of Tie-2, 10  promoting endothelial cell migration, 16  sprouting, 17, 18  and survival 19, 20  in vitro; and increases new vessel growth, branching, maturation, and integrity  in vivo.	bind
37445	2	8771	7	NULL	NULL	0	NULL	statement 1	NULL		induce	NULL				Tie-2	NULL	autophosphorylation of			NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_3_773_s_13	11891175	9, 13- 15  Ang-1 binds and induces autophosphorylation of Tie-2, 10  promoting endothelial cell migration, 16  sprouting, 17, 18  and survival 19, 20  in vitro; and increases new vessel growth, branching, maturation, and integrity  in vivo.	bind
37446	3	8771	7	10	NULL	0	NULL	statement 2	NULL		promote	NULL				endothelial cell 	NULL	migration of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_773_s_13	11891175	9, 13- 15  Ang-1 binds and induces autophosphorylation of Tie-2, 10  promoting endothelial cell migration, 16  sprouting, 17, 18  and survival 19, 20  in vitro; and increases new vessel growth, branching, maturation, and integrity  in vivo.	bind
37447	4	8771	7	NULL	NULL	0	NULL	statement 2	NULL		promote	NULL				endothelial cell	NULL	sprouting of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_773_s_13	11891175	9, 13- 15  Ang-1 binds and induces autophosphorylation of Tie-2, 10  promoting endothelial cell migration, 16  sprouting, 17, 18  and survival 19, 20  in vitro; and increases new vessel growth, branching, maturation, and integrity  in vivo.	bind
37448	5	8771	7	NULL	NULL	0	NULL	statement 2	NULL		promote	NULL				endothelial cell	NULL	survival of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_773_s_13	11891175	9, 13- 15  Ang-1 binds and induces autophosphorylation of Tie-2, 10  promoting endothelial cell migration, 16  sprouting, 17, 18  and survival 19, 20  in vitro; and increases new vessel growth, branching, maturation, and integrity  in vivo.	bind
37449	6	8771	7	NULL	NULL	0	NULL	statement 2	NULL		increase	NULL				new vessel 	NULL	growth of			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_773_s_13	11891175	9, 13- 15  Ang-1 binds and induces autophosphorylation of Tie-2, 10  promoting endothelial cell migration, 16  sprouting, 17, 18  and survival 19, 20  in vitro; and increases new vessel growth, branching, maturation, and integrity  in vivo.	bind
37450	7	8771	7	NULL	NULL	0	NULL	statement 2	NULL		increase	NULL				new vessel	NULL	branching of			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_773_s_13	11891175	9, 13- 15  Ang-1 binds and induces autophosphorylation of Tie-2, 10  promoting endothelial cell migration, 16  sprouting, 17, 18  and survival 19, 20  in vitro; and increases new vessel growth, branching, maturation, and integrity  in vivo.	bind
37451	8	8771	7	NULL	NULL	0	NULL	statement 2	NULL		increase	NULL				new vessel	NULL	maturation of			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_773_s_13	11891175	9, 13- 15  Ang-1 binds and induces autophosphorylation of Tie-2, 10  promoting endothelial cell migration, 16  sprouting, 17, 18  and survival 19, 20  in vitro; and increases new vessel growth, branching, maturation, and integrity  in vivo.	bind
37452	9	8771	7	NULL	NULL	0	NULL	statement 2	NULL		increase	NULL				new vessel	NULL	integrity of			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_amjpathol_160_3_773_s_13	11891175	9, 13- 15  Ang-1 binds and induces autophosphorylation of Tie-2, 10  promoting endothelial cell migration, 16  sprouting, 17, 18  and survival 19, 20  in vitro; and increases new vessel growth, branching, maturation, and integrity  in vivo.	bind
38287	1	8772	5	13	NULL	NULL	NULL	alphavbeta3	GP		is expressed by					melanoma cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_5_1435_s_164	9811334	9, 53 alphavbeta3 expressed by melanoma cells can bind to L1, another member of the Ig gene superfamily found on melanoma cells.	bind
38288	2	8772	5	13	NULL	NULL	NULL	statement 1	GP		bind					L1	GP				NULL	melanoma cells	NULL	NULL	NULL	NULL	gw60_amjpathol_153_5_1435_s_164	9811334	9, 53 alphavbeta3 expressed by melanoma cells can bind to L1, another member of the Ig gene superfamily found on melanoma cells.	bind
38290	3	8772	5	13	NULL	NULL	NULL	L1	GP		is a type of					Ig gene superfamily	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_153_5_1435_s_164	9811334	9, 53 alphavbeta3 expressed by melanoma cells can bind to L1, another member of the Ig gene superfamily found on melanoma cells.	bind
37453	1	8772	7	NULL	NULL	0	NULL	 alphavbeta3 	NULL		bind	NULL				L1	NULL				NULL	melanoma cells	NULL	NULL	NULL	NULL	gw60_amjpathol_153_5_1435_s_164	9811334	9, 53 alphavbeta3 expressed by melanoma cells can bind to L1, another member of the Ig gene superfamily found on melanoma cells.	bind
37454	2	8772	7	NULL	NULL	0	NULL	 alphavbeta3 	NULL		is expressed by	NULL				melanoma cells	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_5_1435_s_164	9811334	9, 53 alphavbeta3 expressed by melanoma cells can bind to L1, another member of the Ig gene superfamily found on melanoma cells.	bind
37455	3	8772	7	NULL	NULL	0	NULL	L1	NULL		is a type of	NULL				Ig gene superfamily	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_153_5_1435_s_164	9811334	9, 53 alphavbeta3 expressed by melanoma cells can bind to L1, another member of the Ig gene superfamily found on melanoma cells.	bind
38291	1	8773	5	13	NULL	NULL	NULL	fVIII	GP		bind					vWf	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_29_18007_s_118	9218428	9, which does not interfere with fVIII binding to vWf ( 19).	bind
37456	1	8773	7	NULL	NULL	0	NULL	fVIII	NULL		bind	NULL				vWf	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_29_18007_s_118	9218428	9, which does not interfere with fVIII binding to vWf ( 19).	bind
38442	1	8774	5	13	NULL	NULL	NULL	cholesterol efflux	Process		is mediated to					apoAI	GP				NULL	macrophages 	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2155_s_29	15358601	9,10  In contrast, unsaturated fatty acids markedly inhibit ABCA1-mediated cholesterol efflux to apoAI in macrophages by increasing ABCA1 turnover and subsequently decreasing cell-surface ABCA1 and apoAI binding to cells.	bind
38443	2	8774	5	13	NULL	NULL	NULL	ABCA1	GP		mediate					statement 1	Process				NULL	macrophages	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2155_s_29	15358601	9,10  In contrast, unsaturated fatty acids markedly inhibit ABCA1-mediated cholesterol efflux to apoAI in macrophages by increasing ABCA1 turnover and subsequently decreasing cell-surface ABCA1 and apoAI binding to cells.	bind
38444	3	8774	5	13	NULL	NULL	NULL	unsaturated fatty acids	Chemical		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2155_s_29	15358601	9,10  In contrast, unsaturated fatty acids markedly inhibit ABCA1-mediated cholesterol efflux to apoAI in macrophages by increasing ABCA1 turnover and subsequently decreasing cell-surface ABCA1 and apoAI binding to cells.	bind
38445	4	8774	5	13	NULL	NULL	NULL	unsaturated fatty acids	Chemical		increase					ABCA1 turnover 	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2155_s_29	15358601	9,10  In contrast, unsaturated fatty acids markedly inhibit ABCA1-mediated cholesterol efflux to apoAI in macrophages by increasing ABCA1 turnover and subsequently decreasing cell-surface ABCA1 and apoAI binding to cells.	bind
38446	5	8774	5	13	NULL	NULL	NULL	ABCA1	GP	cell-surface	bind					cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2155_s_29	15358601	9,10  In contrast, unsaturated fatty acids markedly inhibit ABCA1-mediated cholesterol efflux to apoAI in macrophages by increasing ABCA1 turnover and subsequently decreasing cell-surface ABCA1 and apoAI binding to cells.	bind
38447	6	8774	5	13	NULL	NULL	NULL	apoAI	GP	cell-surface	bind					cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2155_s_29	15358601	9,10  In contrast, unsaturated fatty acids markedly inhibit ABCA1-mediated cholesterol efflux to apoAI in macrophages by increasing ABCA1 turnover and subsequently decreasing cell-surface ABCA1 and apoAI binding to cells.	bind
38448	7	8774	5	13	NULL	NULL	NULL	statement 4	Process		decrease		subsequently			statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2155_s_29	15358601	9,10  In contrast, unsaturated fatty acids markedly inhibit ABCA1-mediated cholesterol efflux to apoAI in macrophages by increasing ABCA1 turnover and subsequently decreasing cell-surface ABCA1 and apoAI binding to cells.	bind
38449	8	8774	5	13	NULL	NULL	NULL	statement 4	Process		decrease		subsequently			statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2155_s_29	15358601	9,10  In contrast, unsaturated fatty acids markedly inhibit ABCA1-mediated cholesterol efflux to apoAI in macrophages by increasing ABCA1 turnover and subsequently decreasing cell-surface ABCA1 and apoAI binding to cells.	bind
37457	1	8774	7	NULL	NULL	0	NULL	cholesterol	NULL		efflux to	NULL				apoAI	NULL				NULL	macrophages	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2155_s_29	15358601	9,10  In contrast, unsaturated fatty acids markedly inhibit ABCA1-mediated cholesterol efflux to apoAI in macrophages by increasing ABCA1 turnover and subsequently decreasing cell-surface ABCA1 and apoAI binding to cells.	bind
37458	2	8774	7	NULL	NULL	0	NULL	ABCA1	NULL		mediates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2155_s_29	15358601	9,10  In contrast, unsaturated fatty acids markedly inhibit ABCA1-mediated cholesterol efflux to apoAI in macrophages by increasing ABCA1 turnover and subsequently decreasing cell-surface ABCA1 and apoAI binding to cells.	bind
37459	3	8774	7	NULL	NULL	0	NULL	unsaturated fatty acids	NULL		inhibit	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2155_s_29	15358601	9,10  In contrast, unsaturated fatty acids markedly inhibit ABCA1-mediated cholesterol efflux to apoAI in macrophages by increasing ABCA1 turnover and subsequently decreasing cell-surface ABCA1 and apoAI binding to cells.	bind
37460	4	8774	7	NULL	NULL	0	NULL	statement 1	NULL		occurs by	NULL				ABCA1	NULL	increase of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2155_s_29	15358601	9,10  In contrast, unsaturated fatty acids markedly inhibit ABCA1-mediated cholesterol efflux to apoAI in macrophages by increasing ABCA1 turnover and subsequently decreasing cell-surface ABCA1 and apoAI binding to cells.	bind
37461	5	8774	7	NULL	NULL	0	NULL	statement 1	NULL		occurs by	NULL				cell surface ABCA1	NULL	decrease of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2155_s_29	15358601	9,10  In contrast, unsaturated fatty acids markedly inhibit ABCA1-mediated cholesterol efflux to apoAI in macrophages by increasing ABCA1 turnover and subsequently decreasing cell-surface ABCA1 and apoAI binding to cells.	bind
37462	6	8774	7	NULL	NULL	0	NULL	apoAI	NULL		bind	NULL				cells	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2155_s_29	15358601	9,10  In contrast, unsaturated fatty acids markedly inhibit ABCA1-mediated cholesterol efflux to apoAI in macrophages by increasing ABCA1 turnover and subsequently decreasing cell-surface ABCA1 and apoAI binding to cells.	bind
37463	7	8774	7	NULL	NULL	0	NULL	statement 1	NULL		occurs by	NULL				statement 6	NULL	decrease of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2155_s_29	15358601	9,10  In contrast, unsaturated fatty acids markedly inhibit ABCA1-mediated cholesterol efflux to apoAI in macrophages by increasing ABCA1 turnover and subsequently decreasing cell-surface ABCA1 and apoAI binding to cells.	bind
56430	8	8774	7	10	NULL	0	NULL	unsaturated fatty acids			increase					ABCA1 turnover					NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_11_2155_s_29	15358601	9,10  In contrast, unsaturated fatty acids markedly inhibit ABCA1-mediated cholesterol efflux to apoAI in macrophages by increasing ABCA1 turnover and subsequently decreasing cell-surface ABCA1 and apoAI binding to cells.	bind
38454	1	8775	5	13	NULL	NULL	NULL	Rho-kinase	GP		is a target protein of		major			small Rho GTPase	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2209_s_24	14592852	9,11 - 15      Rho-kinase, one of the major target proteins of small Rho GTPase, 16,17  was upregulated in spastic coronary segment, leading to an increased phosphorylation of myosin-binding subunit of myosin phosphatase (MLCPh) and the resultant suppression of MLCPh. 11 - 15     Indeed, we recently demonstrated that Rho-kinase is substantially involved in hypercontractions of isolated arteriosclerotic human arteries in vitro 18 as well as in coronary artery spasm of patients with vasospastic angina in vivo.	bind
38455	2	8775	5	13	NULL	NULL	NULL	Rho-kinase	GP		is upregulated in					spastic coronary segment	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2209_s_24	14592852	9,11 - 15      Rho-kinase, one of the major target proteins of small Rho GTPase, 16,17  was upregulated in spastic coronary segment, leading to an increased phosphorylation of myosin-binding subunit of myosin phosphatase (MLCPh) and the resultant suppression of MLCPh. 11 - 15     Indeed, we recently demonstrated that Rho-kinase is substantially involved in hypercontractions of isolated arteriosclerotic human arteries in vitro 18 as well as in coronary artery spasm of patients with vasospastic angina in vivo.	bind
38460	3	8775	5	13	NULL	NULL	NULL	statement 2	Process		increase					MLCPh	GP	phosphorylation of	myosin-binding subunit		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2209_s_24	14592852	9,11 - 15      Rho-kinase, one of the major target proteins of small Rho GTPase, 16,17  was upregulated in spastic coronary segment, leading to an increased phosphorylation of myosin-binding subunit of myosin phosphatase (MLCPh) and the resultant suppression of MLCPh. 11 - 15     Indeed, we recently demonstrated that Rho-kinase is substantially involved in hypercontractions of isolated arteriosclerotic human arteries in vitro 18 as well as in coronary artery spasm of patients with vasospastic angina in vivo.	bind
38462	4	8775	5	13	NULL	NULL	NULL	MLCPh	GP		is					myosin phosphatase	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2209_s_24	14592852	9,11 - 15      Rho-kinase, one of the major target proteins of small Rho GTPase, 16,17  was upregulated in spastic coronary segment, leading to an increased phosphorylation of myosin-binding subunit of myosin phosphatase (MLCPh) and the resultant suppression of MLCPh. 11 - 15     Indeed, we recently demonstrated that Rho-kinase is substantially involved in hypercontractions of isolated arteriosclerotic human arteries in vitro 18 as well as in coronary artery spasm of patients with vasospastic angina in vivo.	bind
38463	5	8775	5	13	NULL	NULL	NULL	statement 3	Process		supress					MLCPh	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2209_s_24	14592852	9,11 - 15      Rho-kinase, one of the major target proteins of small Rho GTPase, 16,17  was upregulated in spastic coronary segment, leading to an increased phosphorylation of myosin-binding subunit of myosin phosphatase (MLCPh) and the resultant suppression of MLCPh. 11 - 15     Indeed, we recently demonstrated that Rho-kinase is substantially involved in hypercontractions of isolated arteriosclerotic human arteries in vitro 18 as well as in coronary artery spasm of patients with vasospastic angina in vivo.	bind
38464	6	8775	5	13	NULL	NULL	NULL	Rho-kinase	GP		is involved in					arteriosclerotic arteries	OrganismPart	hypercontractions of;;isolated;;human			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2209_s_24	14592852	9,11 - 15      Rho-kinase, one of the major target proteins of small Rho GTPase, 16,17  was upregulated in spastic coronary segment, leading to an increased phosphorylation of myosin-binding subunit of myosin phosphatase (MLCPh) and the resultant suppression of MLCPh. 11 - 15     Indeed, we recently demonstrated that Rho-kinase is substantially involved in hypercontractions of isolated arteriosclerotic human arteries in vitro 18 as well as in coronary artery spasm of patients with vasospastic angina in vivo.	bind
38468	7	8775	5	13	NULL	NULL	NULL	Rho-kinase	GP		is involved in					coronary artery spasm	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2209_s_24	14592852	9,11 - 15      Rho-kinase, one of the major target proteins of small Rho GTPase, 16,17  was upregulated in spastic coronary segment, leading to an increased phosphorylation of myosin-binding subunit of myosin phosphatase (MLCPh) and the resultant suppression of MLCPh. 11 - 15     Indeed, we recently demonstrated that Rho-kinase is substantially involved in hypercontractions of isolated arteriosclerotic human arteries in vitro 18 as well as in coronary artery spasm of patients with vasospastic angina in vivo.	bind
46758	8	8775	5	13	NULL	NULL	NULL	statement 7	MedicalFinding		occurs with					vasospastic angina	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2209_s_24	14592852	9,11 - 15      Rho-kinase, one of the major target proteins of small Rho GTPase, 16,17  was upregulated in spastic coronary segment, leading to an increased phosphorylation of myosin-binding subunit of myosin phosphatase (MLCPh) and the resultant suppression of MLCPh. 11 - 15     Indeed, we recently demonstrated that Rho-kinase is substantially involved in hypercontractions of isolated arteriosclerotic human arteries in vitro 18 as well as in coronary artery spasm of patients with vasospastic angina in vivo.	bind
37464	1	8775	7	NULL	NULL	0	NULL	small Rho GTPase	NULL		target	NULL				Rho-kinase	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2209_s_24	14592852	9,11 - 15      Rho-kinase, one of the major target proteins of small Rho GTPase, 16,17  was upregulated in spastic coronary segment, leading to an increased phosphorylation of myosin-binding subunit of myosin phosphatase (MLCPh) and the resultant suppression of MLCPh. 11 - 15     Indeed, we recently demonstrated that Rho-kinase is substantially involved in hypercontractions of isolated arteriosclerotic human arteries in vitro 18 as well as in coronary artery spasm of patients with vasospastic angina in vivo.	bind
37465	2	8775	7	NULL	NULL	0	NULL	Rho-kinase	NULL		is upregulated in	NULL				spastic coronary segment	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2209_s_24	14592852	9,11 - 15      Rho-kinase, one of the major target proteins of small Rho GTPase, 16,17  was upregulated in spastic coronary segment, leading to an increased phosphorylation of myosin-binding subunit of myosin phosphatase (MLCPh) and the resultant suppression of MLCPh. 11 - 15     Indeed, we recently demonstrated that Rho-kinase is substantially involved in hypercontractions of isolated arteriosclerotic human arteries in vitro 18 as well as in coronary artery spasm of patients with vasospastic angina in vivo.	bind
37466	3	8775	7	NULL	NULL	0	NULL	MLCPh	NULL		undergoes	NULL					NULL	phosphorylation of	myosin-binding subunit		NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2209_s_24	14592852	9,11 - 15      Rho-kinase, one of the major target proteins of small Rho GTPase, 16,17  was upregulated in spastic coronary segment, leading to an increased phosphorylation of myosin-binding subunit of myosin phosphatase (MLCPh) and the resultant suppression of MLCPh. 11 - 15     Indeed, we recently demonstrated that Rho-kinase is substantially involved in hypercontractions of isolated arteriosclerotic human arteries in vitro 18 as well as in coronary artery spasm of patients with vasospastic angina in vivo.	bind
37467	4	8775	7	NULL	NULL	0	NULL	statement 2	NULL		increase	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2209_s_24	14592852	9,11 - 15      Rho-kinase, one of the major target proteins of small Rho GTPase, 16,17  was upregulated in spastic coronary segment, leading to an increased phosphorylation of myosin-binding subunit of myosin phosphatase (MLCPh) and the resultant suppression of MLCPh. 11 - 15     Indeed, we recently demonstrated that Rho-kinase is substantially involved in hypercontractions of isolated arteriosclerotic human arteries in vitro 18 as well as in coronary artery spasm of patients with vasospastic angina in vivo.	bind
37468	5	8775	7	NULL	NULL	0	NULL	statement 4	NULL		suppress	NULL				MLCPh	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2209_s_24	14592852	9,11 - 15      Rho-kinase, one of the major target proteins of small Rho GTPase, 16,17  was upregulated in spastic coronary segment, leading to an increased phosphorylation of myosin-binding subunit of myosin phosphatase (MLCPh) and the resultant suppression of MLCPh. 11 - 15     Indeed, we recently demonstrated that Rho-kinase is substantially involved in hypercontractions of isolated arteriosclerotic human arteries in vitro 18 as well as in coronary artery spasm of patients with vasospastic angina in vivo.	bind
37469	6	8775	7	10	NULL	0	NULL	Rho-kinase	NULL		is involved in	NULL	substantially			arteriosclerotic arteries	NULL	hypercontractions of ;; isolated;; human			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2209_s_24	14592852	9,11 - 15      Rho-kinase, one of the major target proteins of small Rho GTPase, 16,17  was upregulated in spastic coronary segment, leading to an increased phosphorylation of myosin-binding subunit of myosin phosphatase (MLCPh) and the resultant suppression of MLCPh. 11 - 15     Indeed, we recently demonstrated that Rho-kinase is substantially involved in hypercontractions of isolated arteriosclerotic human arteries in vitro 18 as well as in coronary artery spasm of patients with vasospastic angina in vivo.	bind
37470	7	8775	7	NULL	NULL	0	NULL	Rho-kinase	NULL		is involved in	NULL				coronary artery spasm	NULL				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2209_s_24	14592852	9,11 - 15      Rho-kinase, one of the major target proteins of small Rho GTPase, 16,17  was upregulated in spastic coronary segment, leading to an increased phosphorylation of myosin-binding subunit of myosin phosphatase (MLCPh) and the resultant suppression of MLCPh. 11 - 15     Indeed, we recently demonstrated that Rho-kinase is substantially involved in hypercontractions of isolated arteriosclerotic human arteries in vitro 18 as well as in coronary artery spasm of patients with vasospastic angina in vivo.	bind
37471	8	8775	7	NULL	NULL	0	NULL	statement 7	NULL		occurs with	NULL				vasospastic angina	NULL				NULL	in vivo	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2209_s_24	14592852	9,11 - 15      Rho-kinase, one of the major target proteins of small Rho GTPase, 16,17  was upregulated in spastic coronary segment, leading to an increased phosphorylation of myosin-binding subunit of myosin phosphatase (MLCPh) and the resultant suppression of MLCPh. 11 - 15     Indeed, we recently demonstrated that Rho-kinase is substantially involved in hypercontractions of isolated arteriosclerotic human arteries in vitro 18 as well as in coronary artery spasm of patients with vasospastic angina in vivo.	bind
37472	9	8775	7	NULL	NULL	0	NULL	MLCPh	NULL		is	NULL				 phosphorylated myosin-binding subunit of myosin phosphatase	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2209_s_24	14592852	9,11 - 15      Rho-kinase, one of the major target proteins of small Rho GTPase, 16,17  was upregulated in spastic coronary segment, leading to an increased phosphorylation of myosin-binding subunit of myosin phosphatase (MLCPh) and the resultant suppression of MLCPh. 11 - 15     Indeed, we recently demonstrated that Rho-kinase is substantially involved in hypercontractions of isolated arteriosclerotic human arteries in vitro 18 as well as in coronary artery spasm of patients with vasospastic angina in vivo.	bind
38470	1	8776	5	13	NULL	NULL	NULL	FAK	GP	activation of	generates					Src family tyrosine kinases	GP	high-affinity binding site to	SH2 domain		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_12_2548_s_39	16195476	9,18,24 - 29        FAK activation generates a high-affinity binding site to the SH2 domain of Src family tyrosine kinases and causes recruitment and activation of Src. 18,19,30   FAK activation also leads to activation of PI3K, which binds to SH2 domain of FAK.	bind
38473	2	8776	5	13	NULL	NULL	NULL	statement 1	GP		recruits					Src	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_12_2548_s_39	16195476	9,18,24 - 29        FAK activation generates a high-affinity binding site to the SH2 domain of Src family tyrosine kinases and causes recruitment and activation of Src. 18,19,30   FAK activation also leads to activation of PI3K, which binds to SH2 domain of FAK.	bind
38476	3	8776	5	13	NULL	NULL	NULL	statement 1	GP		causes					Src	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_12_2548_s_39	16195476	9,18,24 - 29        FAK activation generates a high-affinity binding site to the SH2 domain of Src family tyrosine kinases and causes recruitment and activation of Src. 18,19,30   FAK activation also leads to activation of PI3K, which binds to SH2 domain of FAK.	bind
38479	4	8776	5	13	NULL	NULL	NULL	FAK	GP	activation of	leads to					PI3K	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_12_2548_s_39	16195476	9,18,24 - 29        FAK activation generates a high-affinity binding site to the SH2 domain of Src family tyrosine kinases and causes recruitment and activation of Src. 18,19,30   FAK activation also leads to activation of PI3K, which binds to SH2 domain of FAK.	bind
38480	5	8776	5	13	NULL	NULL	NULL	PI3K	GP		bind					FAK	GP		SH2 domain		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_12_2548_s_39	16195476	9,18,24 - 29        FAK activation generates a high-affinity binding site to the SH2 domain of Src family tyrosine kinases and causes recruitment and activation of Src. 18,19,30   FAK activation also leads to activation of PI3K, which binds to SH2 domain of FAK.	bind
37473	1	8776	7	10	NULL	0	NULL	FAK	NULL	activation of	generates	NULL				Src family tyrosine kinases	NULL	high-affinity binding site to	SH2 domain		NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_12_2548_s_39	16195476	9,18,24 - 29        FAK activation generates a high-affinity binding site to the SH2 domain of Src family tyrosine kinases and causes recruitment and activation of Src. 18,19,30   FAK activation also leads to activation of PI3K, which binds to SH2 domain of FAK.	bind
37474	2	8776	7	NULL	NULL	0	NULL	FAK	NULL	activation of	recruits	NULL				Src	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_12_2548_s_39	16195476	9,18,24 - 29        FAK activation generates a high-affinity binding site to the SH2 domain of Src family tyrosine kinases and causes recruitment and activation of Src. 18,19,30   FAK activation also leads to activation of PI3K, which binds to SH2 domain of FAK.	bind
37475	3	8776	7	NULL	NULL	0	NULL	statement 2	NULL		activates	NULL				Src	NULL				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_12_2548_s_39	16195476	9,18,24 - 29        FAK activation generates a high-affinity binding site to the SH2 domain of Src family tyrosine kinases and causes recruitment and activation of Src. 18,19,30   FAK activation also leads to activation of PI3K, which binds to SH2 domain of FAK.	bind
37476	4	8776	7	NULL	NULL	0	NULL	FAK	NULL	activation of	leads to	NULL				PI3K	NULL	activation of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_12_2548_s_39	16195476	9,18,24 - 29        FAK activation generates a high-affinity binding site to the SH2 domain of Src family tyrosine kinases and causes recruitment and activation of Src. 18,19,30   FAK activation also leads to activation of PI3K, which binds to SH2 domain of FAK.	bind
37477	5	8776	7	NULL	NULL	0	NULL	PI3K 	NULL		binds to	NULL				FAK	NULL		SH2 domain		NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_25_12_2548_s_39	16195476	9,18,24 - 29        FAK activation generates a high-affinity binding site to the SH2 domain of Src family tyrosine kinases and causes recruitment and activation of Src. 18,19,30   FAK activation also leads to activation of PI3K, which binds to SH2 domain of FAK.	bind
38484	1	8777	5	13	NULL	NULL	NULL	9- cis retinoic acid stereoisomer	Chemical		bind					RXR alpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_insectbiochemmolbiol_32_1_33_s_615	11719067	9- cis retinoic acid stereoisomer binds and activates the nuclear receptor RXR alpha.	bind
38485	2	8777	5	13	NULL	NULL	NULL	statement 1	Process		activates					RXR alpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_insectbiochemmolbiol_32_1_33_s_615	11719067	9- cis retinoic acid stereoisomer binds and activates the nuclear receptor RXR alpha.	bind
38486	3	8777	5	13	NULL	NULL	NULL	RXR alpha	GP		is a type of					nuclear receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_insectbiochemmolbiol_32_1_33_s_615	11719067	9- cis retinoic acid stereoisomer binds and activates the nuclear receptor RXR alpha.	bind
37478	1	8777	7	NULL	NULL	0	NULL	9- cis retinoic acid stereoisomer	NULL		binds	NULL				RXR alpha	NULL				NULL		NULL	NULL	NULL	NULL	gw60_insectbiochemmolbiol_32_1_33_s_615	11719067	9- cis retinoic acid stereoisomer binds and activates the nuclear receptor RXR alpha.	bind
37479	2	8777	7	NULL	NULL	0	NULL	statement 1	NULL		activates	NULL				RXR alpha	NULL				NULL		0	NULL	NULL	NULL	gw60_insectbiochemmolbiol_32_1_33_s_615	11719067	9- cis retinoic acid stereoisomer binds and activates the nuclear receptor RXR alpha.	bind
37480	3	8777	7	NULL	NULL	0	NULL	RXR alpha	NULL		is a type of	NULL				nuclear receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_insectbiochemmolbiol_32_1_33_s_615	11719067	9- cis retinoic acid stereoisomer binds and activates the nuclear receptor RXR alpha.	bind
38488	1	8778	5	13	NULL	NULL	NULL	9- Cis-4-oxo-RA	Chemical		bind					RARs	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_pnas_95_26_15424_s_94	9860984	9- Cis-4-oxo-RA binds RARs and RXRs  in vitro	bind
38489	2	8778	5	13	NULL	NULL	NULL	9- Cis-4-oxo-RA	Chemical		bind					RXRs	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_pnas_95_26_15424_s_94	9860984	9- Cis-4-oxo-RA binds RARs and RXRs  in vitro	bind
37481	1	8778	7	NULL	NULL	0	NULL	9- Cis-4-oxo-RA	NULL		binds	NULL				RARs	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_pnas_95_26_15424_s_94	9860984	9- Cis-4-oxo-RA binds RARs and RXRs  in vitro	bind
37482	2	8778	7	NULL	NULL	0	NULL	9- Cis-4-oxo-RA	NULL		binds	NULL				RXRs	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_pnas_95_26_15424_s_94	9860984	9- Cis-4-oxo-RA binds RARs and RXRs  in vitro	bind
38490	1	8779	5	13	NULL	NULL	NULL	9- cis-RA	Chemical		bind					RARs	GP				NULL		NULL	NULL	NULL	NULL	gw60_carcinogenesis_20_2_255_s_161	10069462	9- cis-RA binds both RARs and RXRs, while 4-HPR and probably 2-CPR appear not to bind these receptors ( 40, 41).	bind
38491	2	8779	5	13	NULL	NULL	NULL	9- cis-RA	Chemical		bind					RXRs	GP				NULL		NULL	NULL	NULL	NULL	gw60_carcinogenesis_20_2_255_s_161	10069462	9- cis-RA binds both RARs and RXRs, while 4-HPR and probably 2-CPR appear not to bind these receptors ( 40, 41).	bind
38492	3	8779	5	13	NULL	NULL	NULL	4-HPR	Chemical		does not bind					RARs	GP				NULL		NULL	NULL	NULL	NULL	gw60_carcinogenesis_20_2_255_s_161	10069462	9- cis-RA binds both RARs and RXRs, while 4-HPR and probably 2-CPR appear not to bind these receptors ( 40, 41).	bind
38493	4	8779	5	13	NULL	NULL	NULL	4-HPR	Chemical		does not bind					RXRs	GP				NULL		NULL	NULL	NULL	NULL	gw60_carcinogenesis_20_2_255_s_161	10069462	9- cis-RA binds both RARs and RXRs, while 4-HPR and probably 2-CPR appear not to bind these receptors ( 40, 41).	bind
38494	5	8779	5	13	NULL	NULL	NULL	2-CPR	Chemical		does not bind		probably			RARs	GP				NULL		NULL	NULL	NULL	NULL	gw60_carcinogenesis_20_2_255_s_161	10069462	9- cis-RA binds both RARs and RXRs, while 4-HPR and probably 2-CPR appear not to bind these receptors ( 40, 41).	bind
38495	6	8779	5	13	NULL	NULL	NULL	2-CPR	Chemical		does not bind		probably			RXRs	GP				NULL		NULL	NULL	NULL	NULL	gw60_carcinogenesis_20_2_255_s_161	10069462	9- cis-RA binds both RARs and RXRs, while 4-HPR and probably 2-CPR appear not to bind these receptors ( 40, 41).	bind
37483	1	8779	7	NULL	NULL	0	NULL	9- cis-RA	NULL		binds	NULL				RARs	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_2_255_s_161	10069462	9- cis-RA binds both RARs and RXRs, while 4-HPR and probably 2-CPR appear not to bind these receptors ( 40, 41).	bind
37484	2	8779	7	NULL	NULL	0	NULL	9- cis-RA	NULL		binds	NULL				RXRs	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_2_255_s_161	10069462	9- cis-RA binds both RARs and RXRs, while 4-HPR and probably 2-CPR appear not to bind these receptors ( 40, 41).	bind
37485	3	8779	7	NULL	NULL	0	NULL	4-HPR 	NULL		does not bind	NULL				RARs	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_2_255_s_161	10069462	9- cis-RA binds both RARs and RXRs, while 4-HPR and probably 2-CPR appear not to bind these receptors ( 40, 41).	bind
37486	4	8779	7	NULL	NULL	0	NULL	4-HPR	NULL		does not bind	NULL				RXRs	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_2_255_s_161	10069462	9- cis-RA binds both RARs and RXRs, while 4-HPR and probably 2-CPR appear not to bind these receptors ( 40, 41).	bind
37487	5	8779	7	10	NULL	0	NULL	 2-CPR	NULL		does not bind	NULL	probably			RARs	NULL				NULL		NULL	NULL	NULL	NULL	gw60_carcinogenesis_20_2_255_s_161	10069462	9- cis-RA binds both RARs and RXRs, while 4-HPR and probably 2-CPR appear not to bind these receptors ( 40, 41).	bind
37488	6	8779	7	10	NULL	0	NULL	2-CPR	NULL		does not bind	NULL	probably			RXRs	NULL				NULL		NULL	NULL	NULL	NULL	gw60_carcinogenesis_20_2_255_s_161	10069462	9- cis-RA binds both RARs and RXRs, while 4-HPR and probably 2-CPR appear not to bind these receptors ( 40, 41).	bind
38496	1	8780	5	13	NULL	NULL	NULL	RXR	GP		bind									RXRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_14_8483_s_160	9525962	9- cis-RA increases binding of RXR to an RXRE.	bind
38497	2	8780	5	13	NULL	NULL	NULL	9- cis-RA	Chemical		increase					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_14_8483_s_160	9525962	9- cis-RA increases binding of RXR to an RXRE.	bind
37489	1	8780	7	NULL	NULL	0	NULL	 RXR	NULL		bind	NULL					NULL			RXRE	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8483_s_160	9525962	9- cis-RA increases binding of RXR to an RXRE.	bind
37490	2	8780	7	NULL	NULL	0	NULL	9- cis-RA	NULL		increase	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8483_s_160	9525962	9- cis-RA increases binding of RXR to an RXRE.	bind
38499	1	8781	5	13	NULL	NULL	NULL	9- cis-Retinoic acid stereoisomer	Chemical		bind					RXR	GP				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_7_11_885_s_338	11094341	9- cis-Retinoic acid stereoisomer binds and activates the nuclear receptor RXR .	bind
38500	2	8781	5	13	NULL	NULL	NULL	statement 1	Process		activates					RXR	GP				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_7_11_885_s_338	11094341	9- cis-Retinoic acid stereoisomer binds and activates the nuclear receptor RXR .	bind
38501	3	8781	5	13	NULL	NULL	NULL	RXR	GP		is a type of					nuclear receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_7_11_885_s_338	11094341	9- cis-Retinoic acid stereoisomer binds and activates the nuclear receptor RXR .	bind
37589	1	8781	7	NULL	NULL	0	NULL	9- cis-Retinoic acid stereoisomer	NULL		binds	NULL				RXR	NULL				NULL		0	NULL	NULL	NULL	gw60_chembiol_7_11_885_s_338	11094341	9- cis-Retinoic acid stereoisomer binds and activates the nuclear receptor RXR .	bind
37590	2	8781	7	NULL	NULL	0	NULL	statement 1	NULL		activates	NULL				RXR	NULL				NULL		0	NULL	NULL	NULL	gw60_chembiol_7_11_885_s_338	11094341	9- cis-Retinoic acid stereoisomer binds and activates the nuclear receptor RXR .	bind
37591	3	8781	7	NULL	NULL	0	NULL	RXR	NULL		is a type of	NULL				nuclear receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_chembiol_7_11_885_s_338	11094341	9- cis-Retinoic acid stereoisomer binds and activates the nuclear receptor RXR .	bind
38502	1	8782	5	13	NULL	NULL	NULL	DNA Ligase I	GP		bind					nicked substrates	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_20865_s_139	16731526	9-1-1 Promotes DNA Ligase I Binding to Nicked Substrates --	bind
38503	2	8782	5	13	NULL	NULL	NULL	9-1-1	GP		promotes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_20865_s_139	16731526	9-1-1 Promotes DNA Ligase I Binding to Nicked Substrates --	bind
37592	1	8782	7	NULL	NULL	0	NULL	DNA Ligase I 	NULL		bind	NULL				nicked substrates	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_20865_s_139	16731526	9-1-1 Promotes DNA Ligase I Binding to Nicked Substrates --	bind
46759	2	8782	7	10	NULL	0	NULL	9-1-1	NULL		promotes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_20865_s_139	16731526	9-1-1 Promotes DNA Ligase I Binding to Nicked Substrates --	bind
38507	1	8784	5	13	NULL	NULL	NULL	9-cis retinoic acid stereoisomer	Chemical		bind					RXR	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_68_0_159_s_487	16460270	9-cis retinoic acid stereoisomer binds and activates the nuclear receptor RXR  .	bind
38509	2	8784	5	13	NULL	NULL	NULL	statement 1	Process		activates					RXR	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_68_0_159_s_487	16460270	9-cis retinoic acid stereoisomer binds and activates the nuclear receptor RXR  .	bind
38510	3	8784	5	13	NULL	NULL	NULL	RXR	GP		is a type of					nuclear receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_68_0_159_s_487	16460270	9-cis retinoic acid stereoisomer binds and activates the nuclear receptor RXR  .	bind
38519	1	8788	5	13	NULL	NULL	NULL	estrogen	Chemical		induce					Ov gene	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_37_33890_s_140	12107170	900 (Fig.  4), which contains all the sequences necessary for proper induction of the  Ov gene by estrogen and corticosterone ( 9).	bind
38520	2	8788	5	13	NULL	NULL	NULL	corticosterone	Chemical		induce					Ov gene	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_37_33890_s_140	12107170	900 (Fig.  4), which contains all the sequences necessary for proper induction of the  Ov gene by estrogen and corticosterone ( 9).	bind
37593	1	8788	7	NULL	NULL	0	NULL	estrogen	NULL		induce	NULL				Ov gene	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_37_33890_s_140	12107170	900 (Fig.  4), which contains all the sequences necessary for proper induction of the  Ov gene by estrogen and corticosterone ( 9).	bind
37594	2	8788	7	NULL	NULL	0	NULL	corticosterone	NULL		induce	NULL				Ov gene	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_37_33890_s_140	12107170	900 (Fig.  4), which contains all the sequences necessary for proper induction of the  Ov gene by estrogen and corticosterone ( 9).	bind
38521	1	8789	5	13	NULL	NULL	NULL	tPA	GP		bind					annexin 2	GP	endothelial			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2146_s_153	14551156	91 Concomitant binding of tPA and plasminogen on endothelial annexin 2 results in a 60-fold increase in catalytic efficiency of plasmin generation.	bind
38522	2	8789	5	13	NULL	NULL	NULL	plasminogen	GP		bind					annexin 2	GP	endothelial			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2146_s_153	14551156	91 Concomitant binding of tPA and plasminogen on endothelial annexin 2 results in a 60-fold increase in catalytic efficiency of plasmin generation.	bind
38524	3	8789	5	13	NULL	NULL	NULL	statement 1	Process		increase					plasmin	GP	catalytic efficiency of;; generation of 			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2146_s_153	14551156	91 Concomitant binding of tPA and plasminogen on endothelial annexin 2 results in a 60-fold increase in catalytic efficiency of plasmin generation.	bind
38526	4	8789	5	13	NULL	NULL	NULL	statement 3	Process		increase					plasmin	GP	catalytic efficiency of;;  generation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2146_s_153	14551156	91 Concomitant binding of tPA and plasminogen on endothelial annexin 2 results in a 60-fold increase in catalytic efficiency of plasmin generation.	bind
37595	1	8789	7	10	NULL	0	NULL	 tPA			bind					annexin 2		endothelial 			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2146_s_153	14551156	91 Concomitant binding of tPA and plasminogen on endothelial annexin 2 results in a 60-fold increase in catalytic efficiency of plasmin generation.	bind
37596	2	8789	7	10	NULL	0	NULL	plasminogen			bind					annexin 2		endothelial 			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2146_s_153	14551156	91 Concomitant binding of tPA and plasminogen on endothelial annexin 2 results in a 60-fold increase in catalytic efficiency of plasmin generation.	bind
37597	3	8789	7	10	NULL	0	NULL	statement 1	NULL		increase	NULL				plasmin	NULL	catalytic efficiency of;;  generation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2146_s_153	14551156	91 Concomitant binding of tPA and plasminogen on endothelial annexin 2 results in a 60-fold increase in catalytic efficiency of plasmin generation.	bind
37598	4	8789	7	10	NULL	0	NULL	statement 2	NULL		increase	NULL				plasmin	NULL	catalytic efficiency of;; generation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_12_2146_s_153	14551156	91 Concomitant binding of tPA and plasminogen on endothelial annexin 2 results in a 60-fold increase in catalytic efficiency of plasmin generation.	bind
38529	1	8790	5	13	NULL	NULL	NULL	5''-S DNA	NucleicAcid		bind		covalently						R130K/K167A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_8_5711_s_81	11756402	91% of the input 5''-S DNA was bound covalently by R130K/K167A, and the apparent  kcl of 4.3 x 10 3 s 1 was within a factor of 3 of that of the single K167A mutant on the 5''-S substrate.	bind
37599	1	8790	7	NULL	NULL	0	NULL		NULL		bind	NULL	covalently	 R130K/K167A		5''-S DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_8_5711_s_81	11756402	91% of the input 5''-S DNA was bound covalently by R130K/K167A, and the apparent  kcl of 4.3 x 10 3 s 1 was within a factor of 3 of that of the single K167A mutant on the 5''-S substrate.	bind
38531	1	8791	5	13	NULL	NULL	NULL	c- fos	GP		bind					c- jun	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_8_1882_s_84	10938007	92  AP-1 is a heterodimer of c- fos and c- jun that binds to AP-1 consensus sequences and activates genes related to cell proliferation, migration, apoptosis, and ECM production.	bind
38532	2	8791	5	13	NULL	NULL	NULL	AP-1	GP		is a heterodimer of					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_8_1882_s_84	10938007	92  AP-1 is a heterodimer of c- fos and c- jun that binds to AP-1 consensus sequences and activates genes related to cell proliferation, migration, apoptosis, and ECM production.	bind
38533	3	8791	5	13	NULL	NULL	NULL	AP-1	GP		bind									AP-1 consensus sequences	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_8_1882_s_84	10938007	92  AP-1 is a heterodimer of c- fos and c- jun that binds to AP-1 consensus sequences and activates genes related to cell proliferation, migration, apoptosis, and ECM production.	bind
38535	4	8791	5	13	NULL	NULL	NULL	statement 3	GP		activates					\tcell proliferation genes	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_8_1882_s_84	10938007	92  AP-1 is a heterodimer of c- fos and c- jun that binds to AP-1 consensus sequences and activates genes related to cell proliferation, migration, apoptosis, and ECM production.	bind
38536	5	8791	5	13	NULL	NULL	NULL	statement 3	GP		activates					cell migration genes	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_8_1882_s_84	10938007	92  AP-1 is a heterodimer of c- fos and c- jun that binds to AP-1 consensus sequences and activates genes related to cell proliferation, migration, apoptosis, and ECM production.	bind
38537	6	8791	5	13	NULL	NULL	NULL	statement 3	GP		activates					cell apoptosis genes	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_8_1882_s_84	10938007	92  AP-1 is a heterodimer of c- fos and c- jun that binds to AP-1 consensus sequences and activates genes related to cell proliferation, migration, apoptosis, and ECM production.	bind
38538	7	8791	5	13	NULL	NULL	NULL	statement 3	GP		activates					ECM	GP	production of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_8_1882_s_84	10938007	92  AP-1 is a heterodimer of c- fos and c- jun that binds to AP-1 consensus sequences and activates genes related to cell proliferation, migration, apoptosis, and ECM production.	bind
37650	1	8791	7	10	NULL	0	NULL	c-fos			bind					c-jun					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_8_1882_s_84	10938007	92  AP-1 is a heterodimer of c- fos and c- jun that binds to AP-1 consensus sequences and activates genes related to cell proliferation, migration, apoptosis, and ECM production.	bind
37651	3	8791	7	10	NULL	0	NULL	AP-1			bind									AP-1 consensus sequences	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_8_1882_s_84	10938007	92  AP-1 is a heterodimer of c- fos and c- jun that binds to AP-1 consensus sequences and activates genes related to cell proliferation, migration, apoptosis, and ECM production.	bind
37652	4	8791	7	10	NULL	0	NULL	statement 2			activates					cell proliferation genes					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_8_1882_s_84	10938007	92  AP-1 is a heterodimer of c- fos and c- jun that binds to AP-1 consensus sequences and activates genes related to cell proliferation, migration, apoptosis, and ECM production.	bind
37653	7	8791	7	10	NULL	0	NULL	statement 2			activates					cell migration genes					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_8_1882_s_84	10938007	92  AP-1 is a heterodimer of c- fos and c- jun that binds to AP-1 consensus sequences and activates genes related to cell proliferation, migration, apoptosis, and ECM production.	bind
37654	5	8791	7	NULL	NULL	0	NULL	statement 2	NULL		activates	NULL				cell apoptosis genes	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_8_1882_s_84	10938007	92  AP-1 is a heterodimer of c- fos and c- jun that binds to AP-1 consensus sequences and activates genes related to cell proliferation, migration, apoptosis, and ECM production.	bind
37655	6	8791	7	NULL	NULL	0	NULL	statement 2	NULL		activates	NULL				ECM	NULL	production of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_8_1882_s_84	10938007	92  AP-1 is a heterodimer of c- fos and c- jun that binds to AP-1 consensus sequences and activates genes related to cell proliferation, migration, apoptosis, and ECM production.	bind
56463	2	8791	7	10	NULL	0	NULL	AP-1			is a heterodimer of					statement 1					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_8_1882_s_84	10938007	92  AP-1 is a heterodimer of c- fos and c- jun that binds to AP-1 consensus sequences and activates genes related to cell proliferation, migration, apoptosis, and ECM production.	bind
38547	1	8792	5	13	NULL	NULL	NULL	TSP-1	GP		bind					CD36 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_887_s_148	12067894	92 Binding of TSP-1 to CD36 receptor leads to the recruitment of the Src-related kinase, p59-fyn, and to activation of p38 MAPK.	bind
38549	2	8792	5	13	NULL	NULL	NULL	statement 1	Process		leads to					p59-fyn	GP	recruitment of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_887_s_148	12067894	92 Binding of TSP-1 to CD36 receptor leads to the recruitment of the Src-related kinase, p59-fyn, and to activation of p38 MAPK.	bind
38551	3	8792	5	13	NULL	NULL	NULL	p59-fyn	GP		is a type of					Src-related kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_887_s_148	12067894	92 Binding of TSP-1 to CD36 receptor leads to the recruitment of the Src-related kinase, p59-fyn, and to activation of p38 MAPK.	bind
38552	4	8792	5	13	NULL	NULL	NULL	statement 1	Process		leads to					p38 MAPK	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_887_s_148	12067894	92 Binding of TSP-1 to CD36 receptor leads to the recruitment of the Src-related kinase, p59-fyn, and to activation of p38 MAPK.	bind
37656	1	8792	7	NULL	NULL	0	NULL	TSP-1	NULL		bind	NULL				CD36 receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_887_s_148	12067894	92 Binding of TSP-1 to CD36 receptor leads to the recruitment of the Src-related kinase, p59-fyn, and to activation of p38 MAPK.	bind
37657	2	8792	7	10	NULL	0	NULL	p59-fyn			is a type of					Src-related kinase					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_887_s_148	12067894	92 Binding of TSP-1 to CD36 receptor leads to the recruitment of the Src-related kinase, p59-fyn, and to activation of p38 MAPK.	bind
37658	3	8792	7	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				p59-fyn	NULL	recruitment of 			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_887_s_148	12067894	92 Binding of TSP-1 to CD36 receptor leads to the recruitment of the Src-related kinase, p59-fyn, and to activation of p38 MAPK.	bind
37659	4	8792	7	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				p38 MAPK	NULL	activation of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_6_887_s_148	12067894	92 Binding of TSP-1 to CD36 receptor leads to the recruitment of the Src-related kinase, p59-fyn, and to activation of p38 MAPK.	bind
38554	1	8793	5	13	NULL	NULL	NULL	5''-S DNA	NucleicAcid		bind		covalently						R130K		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_8_5711_s_69	11756402	93% of the input 5''-S DNA was bound covalently by R130K, and the apparent  kcl was 3.7 x 10 2 s 1.	bind
37660	1	8793	7	NULL	NULL	0	NULL		NULL		bind	NULL	covalently	R130K		5''-S DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_8_5711_s_69	11756402	93% of the input 5''-S DNA was bound covalently by R130K, and the apparent  kcl was 3.7 x 10 2 s 1.	bind
38555	1	8794	5	13	NULL	NULL	NULL	Wnt molecules	GP		bind					Fz receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_10_1055_s_150	12039794	94, 95 Binding of the Wnt molecules to Fz receptors activates Dvl, which inhibits the activity of GSK-3beta,  96 thereby stabilizing beta-catenin.	bind
38556	2	8794	5	13	NULL	NULL	NULL	statement 1	Process		activates					Dvl	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_10_1055_s_150	12039794	94, 95 Binding of the Wnt molecules to Fz receptors activates Dvl, which inhibits the activity of GSK-3beta,  96 thereby stabilizing beta-catenin.	bind
38557	3	8794	5	13	NULL	NULL	NULL	statement 2	Process		inhibit					GSK-3beta	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_10_1055_s_150	12039794	94, 95 Binding of the Wnt molecules to Fz receptors activates Dvl, which inhibits the activity of GSK-3beta,  96 thereby stabilizing beta-catenin.	bind
38558	4	8794	5	13	NULL	NULL	NULL	statement 3	Process		stabilize					beta-catenin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_10_1055_s_150	12039794	94, 95 Binding of the Wnt molecules to Fz receptors activates Dvl, which inhibits the activity of GSK-3beta,  96 thereby stabilizing beta-catenin.	bind
37661	1	8794	7	NULL	NULL	0	NULL	Wnt molecules	NULL		bind	NULL				Fz receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_10_1055_s_150	12039794	94, 95 Binding of the Wnt molecules to Fz receptors activates Dvl, which inhibits the activity of GSK-3beta,  96 thereby stabilizing beta-catenin.	bind
37662	2	8794	7	NULL	NULL	0	NULL	statement 1	NULL		activates	NULL				Dvl	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_10_1055_s_150	12039794	94, 95 Binding of the Wnt molecules to Fz receptors activates Dvl, which inhibits the activity of GSK-3beta,  96 thereby stabilizing beta-catenin.	bind
37663	3	8794	7	NULL	NULL	0	NULL	statement 2	NULL		inhibits	NULL				GSK-3beta	NULL	activity of			NULL		0	NULL	NULL	NULL	gw60_circulationres_90_10_1055_s_150	12039794	94, 95 Binding of the Wnt molecules to Fz receptors activates Dvl, which inhibits the activity of GSK-3beta,  96 thereby stabilizing beta-catenin.	bind
37664	4	8794	7	NULL	NULL	0	NULL	statement 3	NULL		stabilize	NULL				beta-catenin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_10_1055_s_150	12039794	94, 95 Binding of the Wnt molecules to Fz receptors activates Dvl, which inhibits the activity of GSK-3beta,  96 thereby stabilizing beta-catenin.	bind
38559	1	8795	5	13	NULL	NULL	NULL	95 kd sperm proteins	GP		bind					ZP3	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_85_5_629_s_136	8646772	95 kd sperm proteins bind ZP3 and serve as tyrosine kinase substrates in response to zona binding.	bind
38561	2	8795	5	13	NULL	NULL	NULL	statement 1	GP		serve as					tyrosine kinase substrates	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_85_5_629_s_136	8646772	95 kd sperm proteins bind ZP3 and serve as tyrosine kinase substrates in response to zona binding.	bind
38563	3	8795	5	13	NULL	NULL	NULL	statement 2	GP		in response to					zona	CellComponent	binding of			NULL		NULL	NULL	NULL	NULL	gw60_cell_85_5_629_s_136	8646772	95 kd sperm proteins bind ZP3 and serve as tyrosine kinase substrates in response to zona binding.	bind
37665	1	8795	7	NULL	NULL	0	NULL	sperm proteins	NULL		bind	NULL				ZP3	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_85_5_629_s_136	8646772	95 kd sperm proteins bind ZP3 and serve as tyrosine kinase substrates in response to zona binding.	bind
37666	2	8795	7	NULL	NULL	0	NULL	statement 1	NULL		serve as	NULL				tyrosine kinase substrates	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_85_5_629_s_136	8646772	95 kd sperm proteins bind ZP3 and serve as tyrosine kinase substrates in response to zona binding.	bind
37667	3	8795	7	NULL	NULL	0	NULL	statement 2	NULL		in response to	NULL				zona	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_cell_85_5_629_s_136	8646772	95 kd sperm proteins bind ZP3 and serve as tyrosine kinase substrates in response to zona binding.	bind
38565	1	8796	5	13	NULL	NULL	NULL	NGF	GP		bind					p75	GP		NTR		NULL	cell lines	NULL	NULL	NULL	NULL	gw60_neuroscience_81_3_861_s_68	9316034	9651 effectively reduces NGF binding to p75NTR on cell lines and on primary rat sympathetic neurons.	bind
38566	2	8796	5	13	NULL	NULL	NULL	NGF	GP		bind					p75	GP		NTR		NULL	primary rat sympathetic neurons	NULL	NULL	NULL	NULL	gw60_neuroscience_81_3_861_s_68	9316034	9651 effectively reduces NGF binding to p75NTR on cell lines and on primary rat sympathetic neurons.	bind
37668	1	8796	7	NULL	NULL	0	NULL	NGF	NULL		bind	NULL				p75	NULL		NTR		NULL	cell lines	0	NULL	NULL	NULL	gw60_neuroscience_81_3_861_s_68	9316034	9651 effectively reduces NGF binding to p75NTR on cell lines and on primary rat sympathetic neurons.	bind
37669	2	8796	7	NULL	NULL	0	NULL	NGF	NULL		bind	NULL				p75	NULL		NTR		NULL	primary rat sympathetic neurons	0	NULL	NULL	NULL	gw60_neuroscience_81_3_861_s_68	9316034	9651 effectively reduces NGF binding to p75NTR on cell lines and on primary rat sympathetic neurons.	bind
38572	1	8797	5	13	NULL	NULL	NULL	nerve growth factor	GP		bind					p75 neurotrophin receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_81_3_861_s_54	9316034	9651 serum and purified 9651 IgG effectively reduce nerve growth factor binding to p75 neurotrophin receptor	bind
38573	2	8797	5	13	NULL	NULL	NULL	9651 serum	OrganismPart		reduces		effectively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_81_3_861_s_54	9316034	9651 serum and purified 9651 IgG effectively reduce nerve growth factor binding to p75 neurotrophin receptor	bind
38574	3	8797	5	13	NULL	NULL	NULL	9651 IgG	GP	purified	reduces		effectively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_81_3_861_s_54	9316034	9651 serum and purified 9651 IgG effectively reduce nerve growth factor binding to p75 neurotrophin receptor	bind
37670	1	8797	7	NULL	NULL	0	NULL	 nerve growth factor	NULL		bind	NULL				p75 neurotrophin receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_neuroscience_81_3_861_s_54	9316034	9651 serum and purified 9651 IgG effectively reduce nerve growth factor binding to p75 neurotrophin receptor	bind
37671	2	8797	7	NULL	NULL	0	NULL	 9651 serum	NULL		reduce	NULL	effectively			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_neuroscience_81_3_861_s_54	9316034	9651 serum and purified 9651 IgG effectively reduce nerve growth factor binding to p75 neurotrophin receptor	bind
37672	3	8797	7	NULL	NULL	0	NULL	9651 IgG	NULL	purified	reduce	NULL	effectively			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_neuroscience_81_3_861_s_54	9316034	9651 serum and purified 9651 IgG effectively reduce nerve growth factor binding to p75 neurotrophin receptor	bind
38575	1	8798	5	13	NULL	NULL	NULL	E-cadherin	GP		bind					cell	Cell				NULL		NULL	NULL	NULL	NULL	gw70_nature_428_6986_950_s_262	15057245	98, 25A (1991)                               Nagafuchi, A. & Takeichi, M. Cell binding function of E-cadherin is regulated  by the cytoplasmic domain.	bind
46760	1	8798	5	13	NULL	NULL	NULL	E-cadherin	GP		regulates			cytoplasmic domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_nature_428_6986_950_s_262	15057245	98, 25A (1991)                               Nagafuchi, A. & Takeichi, M. Cell binding function of E-cadherin is regulated  by the cytoplasmic domain.	bind
37673	1	8798	7	NULL	NULL	0	NULL	E-cadherin	NULL		bind	NULL				Cell	NULL				NULL		0	NULL	NULL	NULL	gw70_nature_428_6986_950_s_262	15057245	98, 25A (1991)                               Nagafuchi, A. & Takeichi, M. Cell binding function of E-cadherin is regulated  by the cytoplasmic domain.	bind
37674	2	8798	7	10	NULL	0	NULL	E-cadherin	NULL		regulates	NULL		cytoplasmic domain		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_nature_428_6986_950_s_262	15057245	98, 25A (1991)                               Nagafuchi, A. & Takeichi, M. Cell binding function of E-cadherin is regulated  by the cytoplasmic domain.	bind
38576	1	8799	5	13	NULL	NULL	NULL	thrombin	GP		bind					subendothelial matrix proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_24_2994_s_171	11413093	99 100  Thrombin also binds to subendothelial matrix proteins, where it is protected from inhibition by heparin.	bind
38577	2	8799	5	13	NULL	NULL	NULL	heparin	Chemical		inhibits					thrombin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_24_2994_s_171	11413093	99 100  Thrombin also binds to subendothelial matrix proteins, where it is protected from inhibition by heparin.	bind
46761	3	8799	5	13	NULL	NULL	NULL	statement 1	Process		leads to					statement 2	Process	protection of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_24_2994_s_171	11413093	99 100  Thrombin also binds to subendothelial matrix proteins, where it is protected from inhibition by heparin.	bind
37675	1	8799	7	NULL	NULL	0	NULL	Thrombin	NULL		binds to	NULL				subendothelial matrix proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_24_2994_s_171	11413093	99 100  Thrombin also binds to subendothelial matrix proteins, where it is protected from inhibition by heparin.	bind
37676	2	8799	7	NULL	NULL	0	NULL	heparin	NULL		inhibits	NULL				thrombin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_103_24_2994_s_171	11413093	99 100  Thrombin also binds to subendothelial matrix proteins, where it is protected from inhibition by heparin.	bind
37677	3	8799	7	10	NULL	0	NULL	statement 1	NULL		leads to	NULL				statement 2	NULL	protection of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_103_24_2994_s_171	11413093	99 100  Thrombin also binds to subendothelial matrix proteins, where it is protected from inhibition by heparin.	bind
38578	1	8800	5	13	NULL	NULL	NULL	GPVI	GP		bind					collagen	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_50_52293_s_134	15466473	9E18 reduced the binding of GPVI to collagen by 45%, reduced the binding of GPVI to CRP by 85%, but had little effect on binding to convulxin (25% inhibition).	bind
38579	2	8800	5	13	NULL	NULL	NULL	9E18	GP		reduce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_50_52293_s_134	15466473	9E18 reduced the binding of GPVI to collagen by 45%, reduced the binding of GPVI to CRP by 85%, but had little effect on binding to convulxin (25% inhibition).	bind
38580	3	8800	5	13	NULL	NULL	NULL	GPVI	GP		bind					CRP	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_50_52293_s_134	15466473	9E18 reduced the binding of GPVI to collagen by 45%, reduced the binding of GPVI to CRP by 85%, but had little effect on binding to convulxin (25% inhibition).	bind
38581	4	8800	5	13	NULL	NULL	NULL	9E18	GP		reduce					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_50_52293_s_134	15466473	9E18 reduced the binding of GPVI to collagen by 45%, reduced the binding of GPVI to CRP by 85%, but had little effect on binding to convulxin (25% inhibition).	bind
38582	5	8800	5	13	NULL	NULL	NULL	GPVI	GP		bind					convulxin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_50_52293_s_134	15466473	9E18 reduced the binding of GPVI to collagen by 45%, reduced the binding of GPVI to CRP by 85%, but had little effect on binding to convulxin (25% inhibition).	bind
38583	6	8800	5	13	NULL	NULL	NULL	9E18	GP		has effect on		little			statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_50_52293_s_134	15466473	9E18 reduced the binding of GPVI to collagen by 45%, reduced the binding of GPVI to CRP by 85%, but had little effect on binding to convulxin (25% inhibition).	bind
37678	1	8800	7	NULL	NULL	0	NULL	GPVI	NULL		bind	NULL				collagen	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_50_52293_s_134	15466473	9E18 reduced the binding of GPVI to collagen by 45%, reduced the binding of GPVI to CRP by 85%, but had little effect on binding to convulxin (25% inhibition).	bind
37679	2	8800	7	NULL	NULL	0	NULL	9E18	NULL		reduce	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_50_52293_s_134	15466473	9E18 reduced the binding of GPVI to collagen by 45%, reduced the binding of GPVI to CRP by 85%, but had little effect on binding to convulxin (25% inhibition).	bind
37680	3	8800	7	NULL	NULL	0	NULL	GPVI	NULL		bind	NULL				CRP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_50_52293_s_134	15466473	9E18 reduced the binding of GPVI to collagen by 45%, reduced the binding of GPVI to CRP by 85%, but had little effect on binding to convulxin (25% inhibition).	bind
37681	4	8800	7	NULL	NULL	0	NULL	9E18	NULL		reduce	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_50_52293_s_134	15466473	9E18 reduced the binding of GPVI to collagen by 45%, reduced the binding of GPVI to CRP by 85%, but had little effect on binding to convulxin (25% inhibition).	bind
37682	5	8800	7	NULL	NULL	0	NULL	GPVI	NULL		bind	NULL				convulxin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_50_52293_s_134	15466473	9E18 reduced the binding of GPVI to collagen by 45%, reduced the binding of GPVI to CRP by 85%, but had little effect on binding to convulxin (25% inhibition).	bind
37683	6	8800	7	10	NULL	0	NULL	9E18	NULL		effect on	NULL	little			statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_50_52293_s_134	15466473	9E18 reduced the binding of GPVI to collagen by 45%, reduced the binding of GPVI to CRP by 85%, but had little effect on binding to convulxin (25% inhibition).	bind
29315	1	8801	6	13	NULL	NULL	NULL	9G8	GP		bind					BSE	GP		Pu1 motif		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_11_7347_s_230	10523623	9G8 binds to the first part of the BSE (Pu1 motif) and stabilizes the binding of the U1 snRNP at the 5' splice site, either directly by interaction with one component of the U1 snRNP or indirectly.	bind
29316	2	8801	6	13	NULL	NULL	NULL	U1 snRNP	GP		bind									5' splice site	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_11_7347_s_230	10523623	9G8 binds to the first part of the BSE (Pu1 motif) and stabilizes the binding of the U1 snRNP at the 5' splice site, either directly by interaction with one component of the U1 snRNP or indirectly.	bind
47529	3	8801	6	13	NULL	NULL	NULL	statement 1	GP		stabilizes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_11_7347_s_230	10523623	9G8 binds to the first part of the BSE (Pu1 motif) and stabilizes the binding of the U1 snRNP at the 5' splice site, either directly by interaction with one component of the U1 snRNP or indirectly.	bind
56160	4	8801	6	13	NULL	NULL	NULL	statement 1	GP		interacts with					U1 snRNP	GP	component of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_11_7347_s_230	10523623	9G8 binds to the first part of the BSE (Pu1 motif) and stabilizes the binding of the U1 snRNP at the 5' splice site, either directly by interaction with one component of the U1 snRNP or indirectly.	bind
56161	5	8801	6	13	NULL	NULL	NULL	statement 1	GP		via		directly			statement 4	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_11_7347_s_230	10523623	9G8 binds to the first part of the BSE (Pu1 motif) and stabilizes the binding of the U1 snRNP at the 5' splice site, either directly by interaction with one component of the U1 snRNP or indirectly.	bind
56162	6	8801	6	13	NULL	NULL	NULL	statement 1	GP		via		indirectly			statement 4	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_11_7347_s_230	10523623	9G8 binds to the first part of the BSE (Pu1 motif) and stabilizes the binding of the U1 snRNP at the 5' splice site, either directly by interaction with one component of the U1 snRNP or indirectly.	bind
56163	7	8801	6	13	NULL	NULL	NULL	statement 5	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_11_7347_s_230	10523623	9G8 binds to the first part of the BSE (Pu1 motif) and stabilizes the binding of the U1 snRNP at the 5' splice site, either directly by interaction with one component of the U1 snRNP or indirectly.	bind
37684	1	8801	7	NULL	NULL	0	NULL	9G8	NULL		binds to	NULL				BSE	NULL		Pu1 motif		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_11_7347_s_230	10523623	9G8 binds to the first part of the BSE (Pu1 motif) and stabilizes the binding of the U1 snRNP at the 5' splice site, either directly by interaction with one component of the U1 snRNP or indirectly.	bind
37685	3	8801	7	NULL	NULL	0	NULL	statement 1	NULL		interacts with	NULL				U1 snRNP	NULL	component of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_11_7347_s_230	10523623	9G8 binds to the first part of the BSE (Pu1 motif) and stabilizes the binding of the U1 snRNP at the 5' splice site, either directly by interaction with one component of the U1 snRNP or indirectly.	bind
37686	2	8801	7	10	NULL	0	NULL	statement 1			stabilizes					statement 7					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_11_7347_s_230	10523623	9G8 binds to the first part of the BSE (Pu1 motif) and stabilizes the binding of the U1 snRNP at the 5' splice site, either directly by interaction with one component of the U1 snRNP or indirectly.	bind
37689	4	8801	7	NULL	NULL	0	NULL	statement 1	NULL		occur via	NULL	directly			statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_11_7347_s_230	10523623	9G8 binds to the first part of the BSE (Pu1 motif) and stabilizes the binding of the U1 snRNP at the 5' splice site, either directly by interaction with one component of the U1 snRNP or indirectly.	bind
47531	5	8801	7	NULL	NULL	0	NULL	statement 1	NULL		occur via	NULL	indirectly			statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_11_7347_s_230	10523623	9G8 binds to the first part of the BSE (Pu1 motif) and stabilizes the binding of the U1 snRNP at the 5' splice site, either directly by interaction with one component of the U1 snRNP or indirectly.	bind
47532	6	8801	7	NULL	NULL	0	NULL	statement 4	NULL		is an alternative to	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_11_7347_s_230	10523623	9G8 binds to the first part of the BSE (Pu1 motif) and stabilizes the binding of the U1 snRNP at the 5' splice site, either directly by interaction with one component of the U1 snRNP or indirectly.	bind
56159	7	8801	7	10	NULL	0	NULL	U1 snRNP			bind									5' splice site	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_11_7347_s_230	10523623	9G8 binds to the first part of the BSE (Pu1 motif) and stabilizes the binding of the U1 snRNP at the 5' splice site, either directly by interaction with one component of the U1 snRNP or indirectly.	bind
29317	1	8802	6	13	NULL	NULL	NULL	9G8	GP		bind					E34	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_1_401_s_172	16249178	9G8 bound to E34 and E3D RNA probes in the presence of the S100 extract and/or Tra2alpha.	bind
29318	2	8802	6	13	NULL	NULL	NULL	9G8	GP		bind					E3D RNA probes	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_1_401_s_172	16249178	9G8 bound to E34 and E3D RNA probes in the presence of the S100 extract and/or Tra2alpha.	bind
29319	3	8802	6	13	NULL	NULL	NULL	statement 1	Process		occurs in presence of					S100 extract	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_1_401_s_172	16249178	9G8 bound to E34 and E3D RNA probes in the presence of the S100 extract and/or Tra2alpha.	bind
29320	4	8802	6	13	NULL	NULL	NULL	statement 1	Process		occurs in presence of					Tra2alpha	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_1_401_s_172	16249178	9G8 bound to E34 and E3D RNA probes in the presence of the S100 extract and/or Tra2alpha.	bind
29321	5	8802	6	13	NULL	NULL	NULL	statement 2	Process		occurs in presence of					S100 extract	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_1_401_s_172	16249178	9G8 bound to E34 and E3D RNA probes in the presence of the S100 extract and/or Tra2alpha.	bind
29322	6	8802	6	13	NULL	NULL	NULL	statement 2	Process		occurs in presence of					Tra2alpha	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_1_401_s_172	16249178	9G8 bound to E34 and E3D RNA probes in the presence of the S100 extract and/or Tra2alpha.	bind
37690	1	8802	7	NULL	NULL	0	NULL	9G8	NULL		bind	NULL				E34 RNA probe	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_401_s_172	16249178	9G8 bound to E34 and E3D RNA probes in the presence of the S100 extract and/or Tra2alpha.	bind
37691	2	8802	7	NULL	NULL	0	NULL	9G8	NULL		bind	NULL				E3D RNA probe	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_401_s_172	16249178	9G8 bound to E34 and E3D RNA probes in the presence of the S100 extract and/or Tra2alpha.	bind
37692	3	8802	7	NULL	NULL	0	NULL	statement 1	NULL		in presence of	NULL				S100 extract	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_401_s_172	16249178	9G8 bound to E34 and E3D RNA probes in the presence of the S100 extract and/or Tra2alpha.	bind
37693	4	8802	7	NULL	NULL	0	NULL	statement 2	NULL		in presence of	NULL				S100 extract	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_401_s_172	16249178	9G8 bound to E34 and E3D RNA probes in the presence of the S100 extract and/or Tra2alpha.	bind
37694	5	8802	7	NULL	NULL	0	NULL	statement 1	NULL		in presence of	NULL				Tra2alpha	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_401_s_172	16249178	9G8 bound to E34 and E3D RNA probes in the presence of the S100 extract and/or Tra2alpha.	bind
37695	6	8802	7	NULL	NULL	0	NULL	statement 2	NULL		in presence of	NULL				Tra2alpha	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_401_s_172	16249178	9G8 bound to E34 and E3D RNA probes in the presence of the S100 extract and/or Tra2alpha.	bind
29323	1	8803	6	13	NULL	NULL	NULL	9G8	GP		bind					E3 RNA probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_1_401_s_158	16249178	9G8 bound to the E3 RNA probe only in the presence of S100 extract ( Fig. 3 B).	bind
29324	2	8803	6	13	NULL	NULL	NULL	statement 1	Process		occurs in presence of					S100 extract	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_1_401_s_158	16249178	9G8 bound to the E3 RNA probe only in the presence of S100 extract ( Fig. 3 B).	bind
37696	1	8803	7	NULL	NULL	0	NULL	9G8	NULL		bind	NULL				E3 RNA probe	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_401_s_158	16249178	9G8 bound to the E3 RNA probe only in the presence of S100 extract ( Fig. 3 B).	bind
37697	2	8803	7	NULL	NULL	0	NULL	statement 1	NULL		in presence of	NULL				S100 extract	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_401_s_158	16249178	9G8 bound to the E3 RNA probe only in the presence of S100 extract ( Fig. 3 B).	bind
29598	1	8804	6	13	NULL	NULL	NULL	9G8	GP		activates 					exon carrying v9b6-5-4 -- 9G8	NucleicAcid	splicing of;; heterologus			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_35_32943_s_264	12826680	9G8, ASF/SF2, and SRp20 Activate Splicing in Vitro of a Heterologous  Exon Carrying v9b6-5-4  -- 9G8, ASF/SF2, and SRp20 bind to v9 exon  sequences, but will this binding activate splicing?	bind
29599	2	8804	6	13	NULL	NULL	NULL	ASF/SF2	GP		activates 					exon carrying ASF/SF2	NucleicAcid	splicing of;; heterologous			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_35_32943_s_264	12826680	9G8, ASF/SF2, and SRp20 Activate Splicing in Vitro of a Heterologous  Exon Carrying v9b6-5-4  -- 9G8, ASF/SF2, and SRp20 bind to v9 exon  sequences, but will this binding activate splicing?	bind
29600	3	8804	6	13	NULL	NULL	NULL	SRp20	GP		activates					exon carrying SRp20	NucleicAcid	splicing of;; heterologous			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_35_32943_s_264	12826680	9G8, ASF/SF2, and SRp20 Activate Splicing in Vitro of a Heterologous  Exon Carrying v9b6-5-4  -- 9G8, ASF/SF2, and SRp20 bind to v9 exon  sequences, but will this binding activate splicing?	bind
47094	4	8804	6	13	NULL	NULL	NULL	9G8	GP		bind					v9 exon sequences	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_35_32943_s_264	12826680	9G8, ASF/SF2, and SRp20 Activate Splicing in Vitro of a Heterologous  Exon Carrying v9b6-5-4  -- 9G8, ASF/SF2, and SRp20 bind to v9 exon  sequences, but will this binding activate splicing?	bind
47095	5	8804	6	13	NULL	NULL	NULL	ASF/SF2	GP		bind					v9 exon sequences	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_35_32943_s_264	12826680	9G8, ASF/SF2, and SRp20 Activate Splicing in Vitro of a Heterologous  Exon Carrying v9b6-5-4  -- 9G8, ASF/SF2, and SRp20 bind to v9 exon  sequences, but will this binding activate splicing?	bind
47096	6	8804	6	13	NULL	NULL	NULL	SRp20	GP		bind					v9 exon sequences	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_35_32943_s_264	12826680	9G8, ASF/SF2, and SRp20 Activate Splicing in Vitro of a Heterologous  Exon Carrying v9b6-5-4  -- 9G8, ASF/SF2, and SRp20 bind to v9 exon  sequences, but will this binding activate splicing?	bind
37698	1	8804	7	10	NULL	0	NULL	9G8	NULL		activate	NULL				 Exon Carrying v9b6-5-4 -- 9G8	NULL	splicing of;;Heterologous			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_35_32943_s_264	12826680	9G8, ASF/SF2, and SRp20 Activate Splicing in Vitro of a Heterologous  Exon Carrying v9b6-5-4  -- 9G8, ASF/SF2, and SRp20 bind to v9 exon  sequences, but will this binding activate splicing?	bind
37699	2	8804	7	10	NULL	0	NULL	ASF/SF2	NULL		activate	NULL				Exon Carrying v9b6-5-4 -- 9G8	NULL	splicing of;;Heterologous			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_35_32943_s_264	12826680	9G8, ASF/SF2, and SRp20 Activate Splicing in Vitro of a Heterologous  Exon Carrying v9b6-5-4  -- 9G8, ASF/SF2, and SRp20 bind to v9 exon  sequences, but will this binding activate splicing?	bind
37700	3	8804	7	10	NULL	0	NULL	SRp20	NULL		activate	NULL				 Exon Carrying v9b6-5-4 -- 9G8	NULL	splicing of;;Heterologous			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_35_32943_s_264	12826680	9G8, ASF/SF2, and SRp20 Activate Splicing in Vitro of a Heterologous  Exon Carrying v9b6-5-4  -- 9G8, ASF/SF2, and SRp20 bind to v9 exon  sequences, but will this binding activate splicing?	bind
37701	4	8804	7	NULL	NULL	0	NULL	9G8	NULL		bind	NULL					NULL			v9 exon sequence	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_35_32943_s_264	12826680	9G8, ASF/SF2, and SRp20 Activate Splicing in Vitro of a Heterologous  Exon Carrying v9b6-5-4  -- 9G8, ASF/SF2, and SRp20 bind to v9 exon  sequences, but will this binding activate splicing?	bind
37702	5	8804	7	NULL	NULL	0	NULL	ASF/SF2	NULL		bind	NULL					NULL			v9 exon sequence	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_35_32943_s_264	12826680	9G8, ASF/SF2, and SRp20 Activate Splicing in Vitro of a Heterologous  Exon Carrying v9b6-5-4  -- 9G8, ASF/SF2, and SRp20 bind to v9 exon  sequences, but will this binding activate splicing?	bind
37703	6	8804	7	NULL	NULL	0	NULL	SRp20	NULL		bind	NULL					NULL			v9 exon sequence	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_35_32943_s_264	12826680	9G8, ASF/SF2, and SRp20 Activate Splicing in Vitro of a Heterologous  Exon Carrying v9b6-5-4  -- 9G8, ASF/SF2, and SRp20 bind to v9 exon  sequences, but will this binding activate splicing?	bind
47538	7	8804	7	NULL	NULL	0	NULL	9G8	NULL		activate	NULL				exon carrying ASF/SF2	NULL	splicing of;;Heterologous			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_35_32943_s_264	12826680	9G8, ASF/SF2, and SRp20 Activate Splicing in Vitro of a Heterologous  Exon Carrying v9b6-5-4  -- 9G8, ASF/SF2, and SRp20 bind to v9 exon  sequences, but will this binding activate splicing?	bind
47539	8	8804	7	NULL	NULL	0	NULL	ASF/SF2	NULL		activate	NULL				exon carrying ASF/SF2	NULL	splicing of;;Heterologous			NULL	in vitro	0	NULL	NULL	NULL	gw70_jbiolchem_278_35_32943_s_264	12826680	9G8, ASF/SF2, and SRp20 Activate Splicing in Vitro of a Heterologous  Exon Carrying v9b6-5-4  -- 9G8, ASF/SF2, and SRp20 bind to v9 exon  sequences, but will this binding activate splicing?	bind
47540	9	8804	7	NULL	NULL	0	NULL	SRp20	NULL		activate	NULL				exon carrying ASF/SF2	NULL	splicing of;;Heterologous			NULL	in vitro	0	NULL	NULL	NULL	gw70_jbiolchem_278_35_32943_s_264	12826680	9G8, ASF/SF2, and SRp20 Activate Splicing in Vitro of a Heterologous  Exon Carrying v9b6-5-4  -- 9G8, ASF/SF2, and SRp20 bind to v9 exon  sequences, but will this binding activate splicing?	bind
47541	10	8804	7	NULL	NULL	0	NULL	9G8	NULL		activate	NULL				exon carrying SRp20	NULL	splicing of;;Heterologous			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_35_32943_s_264	12826680	9G8, ASF/SF2, and SRp20 Activate Splicing in Vitro of a Heterologous  Exon Carrying v9b6-5-4  -- 9G8, ASF/SF2, and SRp20 bind to v9 exon  sequences, but will this binding activate splicing?	bind
47542	11	8804	7	NULL	NULL	0	NULL	ASF/SF2	NULL		activate	NULL				exon carrying SRp20	NULL	splicing of;;Heterologous			NULL	in vitro	0	NULL	NULL	NULL	gw70_jbiolchem_278_35_32943_s_264	12826680	9G8, ASF/SF2, and SRp20 Activate Splicing in Vitro of a Heterologous  Exon Carrying v9b6-5-4  -- 9G8, ASF/SF2, and SRp20 bind to v9 exon  sequences, but will this binding activate splicing?	bind
47543	12	8804	7	NULL	NULL	0	NULL	 SRp20	NULL		activate	NULL				exon carrying SRp20	NULL	splicing of;;Heterologous			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_35_32943_s_264	12826680	9G8, ASF/SF2, and SRp20 Activate Splicing in Vitro of a Heterologous  Exon Carrying v9b6-5-4  -- 9G8, ASF/SF2, and SRp20 bind to v9 exon  sequences, but will this binding activate splicing?	bind
29325	1	8805	6	13	NULL	NULL	NULL	Tdp-ICL	NucleicAcid		bind					XPC-hHR23B	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_9_2993_s_157	15914671	: RPA-Tdp-ICL super-shifted complex also migrated at the same position as when Tdp-ICL  was bound by XPC-hHR23B.	bind
37704	1	8805	7	NULL	NULL	0	NULL	XPC-hHR23B	NULL		bind	NULL				Tdp-ICL	NULL				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_9_2993_s_157	15914671	: RPA-Tdp-ICL super-shifted complex also migrated at the same position as when Tdp-ICL  was bound by XPC-hHR23B.	bind
29326	1	8806	6	13	NULL	NULL	NULL	Cl-	Chemical		bind					cyt bo3 plus NO2	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_5_1272_s_107	12207912	; and cyt  bo3 (~7  M) plus NO2- (10 mM) (- - -), and Cl- bound cyt  bo3 plus NO2- (-.	bind
37914	1	8806	7	NULL	NULL	0	NULL	 Cl-	NULL		bind	NULL				cyt bo3 plus NO2	NULL				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_5_1272_s_107	12207912	; and cyt  bo3 (~7  M) plus NO2- (10 mM) (- - -), and Cl- bound cyt  bo3 plus NO2- (-.	bind
29327	1	8807	6	13	NULL	NULL	NULL	XylR protein	GP		bind					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_annurevmicrobiol_51_0_341_s_294	9343354	A   ascade of Events Leading to Coordinate Expression of Upper and  Meta   Pathways    After binding an effector, the XylR protein binds ATP and oligomerizes   and undergoes a series of conformational changes that lead to a state   with enhanced ATPase activity that is active, from a transcriptional   point of view ( 104,  105).	bind
29328	3	8807	6	13	NULL	NULL	NULL	statement 2	Process		leads to					ATPase activity	Process	enhanced			NULL		NULL	NULL	NULL	NULL	gw60_annurevmicrobiol_51_0_341_s_294	9343354	A   ascade of Events Leading to Coordinate Expression of Upper and  Meta   Pathways    After binding an effector, the XylR protein binds ATP and oligomerizes   and undergoes a series of conformational changes that lead to a state   with enhanced ATPase activity that is active, from a transcriptional   point of view ( 104,  105).	bind
46904	4	8807	6	13	NULL	NULL	NULL	effector	GP	binding of	leads to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_annurevmicrobiol_51_0_341_s_294	9343354	A   ascade of Events Leading to Coordinate Expression of Upper and  Meta   Pathways    After binding an effector, the XylR protein binds ATP and oligomerizes   and undergoes a series of conformational changes that lead to a state   with enhanced ATPase activity that is active, from a transcriptional   point of view ( 104,  105).	bind
56164	2	8807	6	13	NULL	NULL	NULL	statement 1	GP		oligomerize					XylR protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_annurevmicrobiol_51_0_341_s_294	9343354	A   ascade of Events Leading to Coordinate Expression of Upper and  Meta   Pathways    After binding an effector, the XylR protein binds ATP and oligomerizes   and undergoes a series of conformational changes that lead to a state   with enhanced ATPase activity that is active, from a transcriptional   point of view ( 104,  105).	bind
37915	1	8807	7	NULL	NULL	0	NULL	XylR protein 	NULL		binds	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw60_annurevmicrobiol_51_0_341_s_294	9343354	A   ascade of Events Leading to Coordinate Expression of Upper and  Meta   Pathways    After binding an effector, the XylR protein binds ATP and oligomerizes   and undergoes a series of conformational changes that lead to a state   with enhanced ATPase activity that is active, from a transcriptional   point of view ( 104,  105).	bind
37916	2	8807	7	NULL	NULL	0	NULL	statement 1	NULL		oligomerize	NULL				XylR protein 	NULL				NULL		0	NULL	NULL	NULL	gw60_annurevmicrobiol_51_0_341_s_294	9343354	A   ascade of Events Leading to Coordinate Expression of Upper and  Meta   Pathways    After binding an effector, the XylR protein binds ATP and oligomerizes   and undergoes a series of conformational changes that lead to a state   with enhanced ATPase activity that is active, from a transcriptional   point of view ( 104,  105).	bind
37919	3	8807	7	10	NULL	0	NULL	statement 2			enhance					ATPase activity					NULL		NULL	NULL	NULL	NULL	gw60_annurevmicrobiol_51_0_341_s_294	9343354	A   ascade of Events Leading to Coordinate Expression of Upper and  Meta   Pathways    After binding an effector, the XylR protein binds ATP and oligomerizes   and undergoes a series of conformational changes that lead to a state   with enhanced ATPase activity that is active, from a transcriptional   point of view ( 104,  105).	bind
37921	4	8807	7	10	NULL	0	NULL	statement 1			occurs after					effector		binding of			NULL		NULL	NULL	NULL	NULL	gw60_annurevmicrobiol_51_0_341_s_294	9343354	A   ascade of Events Leading to Coordinate Expression of Upper and  Meta   Pathways    After binding an effector, the XylR protein binds ATP and oligomerizes   and undergoes a series of conformational changes that lead to a state   with enhanced ATPase activity that is active, from a transcriptional   point of view ( 104,  105).	bind
29329	1	8808	6	13	NULL	NULL	NULL	neurotractin	GP		bind					CEPU-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_4_865_s_264	10330412	A   KD of 3 x 10 8 M was measured for the binding of neurotractin to the GPI-linked molecule CEPU-1 (Fig.  7), an  affinity that is lower than that usually reported for soluble  polypeptide ligands that bind to cell surface receptors, for  instance the neurotrophins (Dechant et al., 1994  ).	bind
29330	2	8808	6	13	NULL	NULL	NULL	CEPU-1	GP		is a type of					GPI-linked molecule	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_4_865_s_264	10330412	A   KD of 3 x 10 8 M was measured for the binding of neurotractin to the GPI-linked molecule CEPU-1 (Fig.  7), an  affinity that is lower than that usually reported for soluble  polypeptide ligands that bind to cell surface receptors, for  instance the neurotrophins (Dechant et al., 1994  ).	bind
29331	3	8808	6	13	NULL	NULL	NULL	polypeptide ligands	GP	soluble	bind					neurotrophins	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_4_865_s_264	10330412	A   KD of 3 x 10 8 M was measured for the binding of neurotractin to the GPI-linked molecule CEPU-1 (Fig.  7), an  affinity that is lower than that usually reported for soluble  polypeptide ligands that bind to cell surface receptors, for  instance the neurotrophins (Dechant et al., 1994  ).	bind
29332	4	8808	6	13	NULL	NULL	NULL	neurotrophins	GP		is a type of					cell-surface receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_4_865_s_264	10330412	A   KD of 3 x 10 8 M was measured for the binding of neurotractin to the GPI-linked molecule CEPU-1 (Fig.  7), an  affinity that is lower than that usually reported for soluble  polypeptide ligands that bind to cell surface receptors, for  instance the neurotrophins (Dechant et al., 1994  ).	bind
29333	5	8808	6	13	NULL	NULL	NULL	statement 1	Process	affinity of	is lower than					statement 3	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_4_865_s_264	10330412	A   KD of 3 x 10 8 M was measured for the binding of neurotractin to the GPI-linked molecule CEPU-1 (Fig.  7), an  affinity that is lower than that usually reported for soluble  polypeptide ligands that bind to cell surface receptors, for  instance the neurotrophins (Dechant et al., 1994  ).	bind
37922	1	8808	7	NULL	NULL	0	NULL	neurotractin	NULL		bind	NULL				CEPU-1	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_4_865_s_264	10330412	A   KD of 3 x 10 8 M was measured for the binding of neurotractin to the GPI-linked molecule CEPU-1 (Fig.  7), an  affinity that is lower than that usually reported for soluble  polypeptide ligands that bind to cell surface receptors, for  instance the neurotrophins (Dechant et al., 1994  ).	bind
37925	2	8808	7	NULL	NULL	0	NULL	polypeptide ligands 	NULL	soluble	binds to	NULL				neurotrophins	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_4_865_s_264	10330412	A   KD of 3 x 10 8 M was measured for the binding of neurotractin to the GPI-linked molecule CEPU-1 (Fig.  7), an  affinity that is lower than that usually reported for soluble  polypeptide ligands that bind to cell surface receptors, for  instance the neurotrophins (Dechant et al., 1994  ).	bind
37926	3	8808	7	NULL	NULL	0	NULL	CEPU-1	NULL		is a type of	NULL				GPI-linked molecule	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_4_865_s_264	10330412	A   KD of 3 x 10 8 M was measured for the binding of neurotractin to the GPI-linked molecule CEPU-1 (Fig.  7), an  affinity that is lower than that usually reported for soluble  polypeptide ligands that bind to cell surface receptors, for  instance the neurotrophins (Dechant et al., 1994  ).	bind
37949	4	8808	7	NULL	NULL	0	NULL	 neurotrophins	NULL		is a type of	NULL				cell surface receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_4_865_s_264	10330412	A   KD of 3 x 10 8 M was measured for the binding of neurotractin to the GPI-linked molecule CEPU-1 (Fig.  7), an  affinity that is lower than that usually reported for soluble  polypeptide ligands that bind to cell surface receptors, for  instance the neurotrophins (Dechant et al., 1994  ).	bind
37950	5	8808	7	NULL	NULL	0	NULL	statement 1	NULL	affinity of	is lower than	NULL				statement 2	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_4_865_s_264	10330412	A   KD of 3 x 10 8 M was measured for the binding of neurotractin to the GPI-linked molecule CEPU-1 (Fig.  7), an  affinity that is lower than that usually reported for soluble  polypeptide ligands that bind to cell surface receptors, for  instance the neurotrophins (Dechant et al., 1994  ).	bind
29335	1	8809	6	13	NULL	NULL	NULL	EGF ligand	GP		bind					EGFR	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1673_3_186_s_227	15279890	A   trans mechanism explains the activation of ErbB-2 in the cells by EGF, a ligand that binds  EGFR, but not ErbB-2.	bind
29336	2	8809	6	13	NULL	NULL	NULL	EGF ligand	GP		does not bind					ErbB-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1673_3_186_s_227	15279890	A   trans mechanism explains the activation of ErbB-2 in the cells by EGF, a ligand that binds  EGFR, but not ErbB-2.	bind
46943	3	8809	6	13	NULL	NULL	NULL	EGF ligand	GP		activates					ErbB-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1673_3_186_s_227	15279890	A   trans mechanism explains the activation of ErbB-2 in the cells by EGF, a ligand that binds  EGFR, but not ErbB-2.	bind
46944	4	8809	6	13	NULL	NULL	NULL	statement 3	Process		via					trans mechanism	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1673_3_186_s_227	15279890	A   trans mechanism explains the activation of ErbB-2 in the cells by EGF, a ligand that binds  EGFR, but not ErbB-2.	bind
37951	1	8809	7	10	NULL	0	NULL	EGF ligand	NULL		activates	NULL				ErbB-2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1673_3_186_s_227	15279890	A   trans mechanism explains the activation of ErbB-2 in the cells by EGF, a ligand that binds  EGFR, but not ErbB-2.	bind
37952	2	8809	7	10	NULL	0	NULL	EGF ligand	NULL		binds	NULL				EGFR	NULL				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1673_3_186_s_227	15279890	A   trans mechanism explains the activation of ErbB-2 in the cells by EGF, a ligand that binds  EGFR, but not ErbB-2.	bind
37953	3	8809	7	10	NULL	0	NULL	EGF ligand	NULL		does not bind	NULL				ErbB-2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1673_3_186_s_227	15279890	A   trans mechanism explains the activation of ErbB-2 in the cells by EGF, a ligand that binds  EGFR, but not ErbB-2.	bind
42308	4	8809	7	NULL	NULL	0	NULL	statement 1	NULL		via	NULL				trans mechanism	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1673_3_186_s_227	15279890	A   trans mechanism explains the activation of ErbB-2 in the cells by EGF, a ligand that binds  EGFR, but not ErbB-2.	bind
29337	1	8810	6	13	NULL	NULL	NULL	interferon-induced factor	GP		bind					H-2Kb gene	GP			interferon response sequence	NULL		NULL	NULL	NULL	NULL	gw60_immunity_5_4_365_s_384	8885869	A  -interferon-induced factor that binds the interferon response sequence of the MHC class I gene, H-2Kb.	bind
29338	2	8810	6	13	NULL	NULL	NULL	H-2Kb	GP		is a type of					MHC class I gene	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_5_4_365_s_384	8885869	A  -interferon-induced factor that binds the interferon response sequence of the MHC class I gene, H-2Kb.	bind
37954	1	8810	7	NULL	NULL	0	NULL	interferon-induced factor	NULL		binds to	NULL				H-2Kb	NULL			interferon response sequence	NULL		0	NULL	NULL	NULL	gw60_immunity_5_4_365_s_384	8885869	A  -interferon-induced factor that binds the interferon response sequence of the MHC class I gene, H-2Kb.	bind
37955	2	8810	7	NULL	NULL	0	NULL	H-2Kb	NULL		is a type of	NULL				MHC class I  gene	NULL				NULL		0	NULL	NULL	NULL	gw60_immunity_5_4_365_s_384	8885869	A  -interferon-induced factor that binds the interferon response sequence of the MHC class I gene, H-2Kb.	bind
29339	1	8811	6	13	NULL	NULL	NULL	Cbl	GP		bind		high affinity			Crk	GP		SH2 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_14_8435_s_71	8626543	A  20-fold shorter exposure of this blot emphasizes the markedly higher  binding of Cbl to Crk SH2 ( Fig. 1  A,  middle  panel).	bind
37958	1	8811	7	NULL	NULL	0	NULL	 Cbl	NULL		bind	NULL				Crk	NULL		SH2		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8435_s_71	8626543	A  20-fold shorter exposure of this blot emphasizes the markedly higher  binding of Cbl to Crk SH2 ( Fig. 1  A,  middle  panel).	bind
29340	1	8812	6	13	NULL	NULL	NULL	DnaJ	GP		bind					DnaK	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_11_6137_s_84	8626401	A  4-fold decrease in DnaJ concentration decreased in half the  DnaJ-dependent effect on DnaK's fluorescence (result not shown),  suggesting that binding of DnaJ to DnaK is the rate-limiting step.	bind
37960	1	8812	7	NULL	NULL	0	NULL	DnaJ 	NULL		bind	NULL				DnaK	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_11_6137_s_84	8626401	A  4-fold decrease in DnaJ concentration decreased in half the  DnaJ-dependent effect on DnaK's fluorescence (result not shown),  suggesting that binding of DnaJ to DnaK is the rate-limiting step.	bind
47111	1	8813	6	13	NULL	NULL	NULL	MCF-7	Cell		bind					nuclear protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_23_20490_s_116	12657623	A  50-molar excess of cold  - 1575G oligonucleotide strongly competed for  MCF-7 nuclear protein binding, resulting in the disappearance of the major  shifted complex ( Fig. 3,  lane 3), whereas a 50-molar excess of cold  - 1575A  oligonucleotide revealed only partial competition  ( Fig. 3,  lane 4).	bind
47112	2	8813	6	13	NULL	NULL	NULL	oligonucleotide	NucleicAcid		bind				1575G	nuclear protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_23_20490_s_116	12657623	A  50-molar excess of cold  - 1575G oligonucleotide strongly competed for  MCF-7 nuclear protein binding, resulting in the disappearance of the major  shifted complex ( Fig. 3,  lane 3), whereas a 50-molar excess of cold  - 1575A  oligonucleotide revealed only partial competition  ( Fig. 3,  lane 4).	bind
47113	3	8813	6	13	NULL	NULL	NULL	oligonucleotide	NucleicAcid		bind				1575A	nuclear protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_23_20490_s_116	12657623	A  50-molar excess of cold  - 1575G oligonucleotide strongly competed for  MCF-7 nuclear protein binding, resulting in the disappearance of the major  shifted complex ( Fig. 3,  lane 3), whereas a 50-molar excess of cold  - 1575A  oligonucleotide revealed only partial competition  ( Fig. 3,  lane 4).	bind
47114	4	8813	6	13	NULL	NULL	NULL	statement 1	Process		competes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_23_20490_s_116	12657623	A  50-molar excess of cold  - 1575G oligonucleotide strongly competed for  MCF-7 nuclear protein binding, resulting in the disappearance of the major  shifted complex ( Fig. 3,  lane 3), whereas a 50-molar excess of cold  - 1575A  oligonucleotide revealed only partial competition  ( Fig. 3,  lane 4).	bind
47115	5	8813	6	13	NULL	NULL	NULL	statement 1	Process		competes		partially			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_23_20490_s_116	12657623	A  50-molar excess of cold  - 1575G oligonucleotide strongly competed for  MCF-7 nuclear protein binding, resulting in the disappearance of the major  shifted complex ( Fig. 3,  lane 3), whereas a 50-molar excess of cold  - 1575A  oligonucleotide revealed only partial competition  ( Fig. 3,  lane 4).	bind
37966	1	8813	7	NULL	NULL	0	NULL	MCF-7	NULL		bind	NULL				nuclear protein	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_23_20490_s_116	12657623	A  50-molar excess of cold  - 1575G oligonucleotide strongly competed for  MCF-7 nuclear protein binding, resulting in the disappearance of the major  shifted complex ( Fig. 3,  lane 3), whereas a 50-molar excess of cold  - 1575A  oligonucleotide revealed only partial competition  ( Fig. 3,  lane 4).	bind
37967	2	8813	7	NULL	NULL	0	NULL	oligonucleotide	NULL		bind	NULL			1575G	nuclear protein	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_23_20490_s_116	12657623	A  50-molar excess of cold  - 1575G oligonucleotide strongly competed for  MCF-7 nuclear protein binding, resulting in the disappearance of the major  shifted complex ( Fig. 3,  lane 3), whereas a 50-molar excess of cold  - 1575A  oligonucleotide revealed only partial competition  ( Fig. 3,  lane 4).	bind
37968	3	8813	7	NULL	NULL	0	NULL	oligonucleotide	NULL		bind	NULL			1575A	nuclear protein	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_23_20490_s_116	12657623	A  50-molar excess of cold  - 1575G oligonucleotide strongly competed for  MCF-7 nuclear protein binding, resulting in the disappearance of the major  shifted complex ( Fig. 3,  lane 3), whereas a 50-molar excess of cold  - 1575A  oligonucleotide revealed only partial competition  ( Fig. 3,  lane 4).	bind
42309	4	8813	7	NULL	NULL	0	NULL	statement 2 	NULL		compete with	NULL	strongly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_23_20490_s_116	12657623	A  50-molar excess of cold  - 1575G oligonucleotide strongly competed for  MCF-7 nuclear protein binding, resulting in the disappearance of the major  shifted complex ( Fig. 3,  lane 3), whereas a 50-molar excess of cold  - 1575A  oligonucleotide revealed only partial competition  ( Fig. 3,  lane 4).	bind
42310	5	8813	7	NULL	NULL	0	NULL	statement 3	NULL		compete with	NULL	partially			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_23_20490_s_116	12657623	A  50-molar excess of cold  - 1575G oligonucleotide strongly competed for  MCF-7 nuclear protein binding, resulting in the disappearance of the major  shifted complex ( Fig. 3,  lane 3), whereas a 50-molar excess of cold  - 1575A  oligonucleotide revealed only partial competition  ( Fig. 3,  lane 4).	bind
29382	1	8814	6	13	NULL	NULL	NULL	Gbeta	GP		bind					CIR	GP	recombinant			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_49_29059_s_81	7493925	A  and  B  demonstrate the specificity  of Gbeta   binding to recombinant CIR ( rCIR) or to  recombinant GIRK1 ( rGIRK1).	bind
29383	2	8814	6	13	NULL	NULL	NULL	Gbeta	GP		bind					GIRK1	GP	recombinant			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_49_29059_s_81	7493925	A  and  B  demonstrate the specificity  of Gbeta   binding to recombinant CIR ( rCIR) or to  recombinant GIRK1 ( rGIRK1).	bind
29384	3	8814	6	13	NULL	NULL	NULL	recombinant CIR	GP		is					rCIR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_49_29059_s_81	7493925	A  and  B  demonstrate the specificity  of Gbeta   binding to recombinant CIR ( rCIR) or to  recombinant GIRK1 ( rGIRK1).	bind
29385	4	8814	6	13	NULL	NULL	NULL	recombinant GIRK1	GP		is					rGIRK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_49_29059_s_81	7493925	A  and  B  demonstrate the specificity  of Gbeta   binding to recombinant CIR ( rCIR) or to  recombinant GIRK1 ( rGIRK1).	bind
37969	1	8814	7	NULL	NULL	0	NULL	Gbeta	NULL		bind	NULL				rCIR	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_49_29059_s_81	7493925	A  and  B  demonstrate the specificity  of Gbeta   binding to recombinant CIR ( rCIR) or to  recombinant GIRK1 ( rGIRK1).	bind
37970	2	8814	7	NULL	NULL	0	NULL	Gbeta	NULL		bind	NULL				 rGIRK1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_49_29059_s_81	7493925	A  and  B  demonstrate the specificity  of Gbeta   binding to recombinant CIR ( rCIR) or to  recombinant GIRK1 ( rGIRK1).	bind
37971	3	8814	7	NULL	NULL	0	NULL	rCIR	NULL		is	NULL				recombinant CIR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_49_29059_s_81	7493925	A  and  B  demonstrate the specificity  of Gbeta   binding to recombinant CIR ( rCIR) or to  recombinant GIRK1 ( rGIRK1).	bind
37972	4	8814	7	NULL	NULL	0	NULL	 rGIRK1	NULL		is	NULL				recombinant  GIRK1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_49_29059_s_81	7493925	A  and  B  demonstrate the specificity  of Gbeta   binding to recombinant CIR ( rCIR) or to  recombinant GIRK1 ( rGIRK1).	bind
29392	1	8815	6	13	NULL	NULL	NULL	tropomyosin	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_14_7836_s_64	7713874	A  and  B  show that tropomyosin was bound to the actin    in both  the undiluted (100 nM  actin +  100 nM  tropomyosin) and the 10-fold diluted samples, respectively.	bind
37973	1	8815	7	NULL	NULL	0	NULL	tropomyosin	NULL		bind	NULL				actin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_14_7836_s_64	7713874	A  and  B  show that tropomyosin was bound to the actin    in both  the undiluted (100 nM  actin +  100 nM  tropomyosin) and the 10-fold diluted samples, respectively.	bind
29393	1	8816	6	13	NULL	NULL	NULL	Arg molecule	AminoAcid		bind					substrate binding helix	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_34_24100_s_58	10446182	A  blue Arg molecule is also shown bound to the substrate-binding helix and positioned  above the  red heme group contained in this subunit of the dimer.	bind
37974	1	8816	7	NULL	NULL	0	NULL	Arg molecule	NULL		bind	NULL				substrate-binding helix	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_34_24100_s_58	10446182	A  blue Arg molecule is also shown bound to the substrate-binding helix and positioned  above the  red heme group contained in this subunit of the dimer.	bind
29395	1	8817	6	13	NULL	NULL	NULL	cdc24	GP		bind					Rsr1/Bud1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_13_13084_s_298	15657049	A  bud1 null mutant is able to respond to mating pheromone and to form shmoos ( ,  ), suggesting that the defect in Ste5 recruitment is not linked to a defect in Cdc24 binding to Rsr1/Bud1.	bind
29396	2	8817	6	13	NULL	NULL	NULL	bud1	GP	null mutant	respond to					mating pheromone	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_13_13084_s_298	15657049	A  bud1 null mutant is able to respond to mating pheromone and to form shmoos ( ,  ), suggesting that the defect in Ste5 recruitment is not linked to a defect in Cdc24 binding to Rsr1/Bud1.	bind
46945	3	8817	6	13	NULL	NULL	NULL	statement 2	Process		forms					shmoos	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_13_13084_s_298	15657049	A  bud1 null mutant is able to respond to mating pheromone and to form shmoos ( ,  ), suggesting that the defect in Ste5 recruitment is not linked to a defect in Cdc24 binding to Rsr1/Bud1.	bind
46946	4	8817	6	13	NULL	NULL	NULL	Ste5	GP	\tdefect in recruitment of	is not linked to					statement 1	Process	defect in			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_13_13084_s_298	15657049	A  bud1 null mutant is able to respond to mating pheromone and to form shmoos ( ,  ), suggesting that the defect in Ste5 recruitment is not linked to a defect in Cdc24 binding to Rsr1/Bud1.	bind
37975	1	8817	7	NULL	NULL	0	NULL	 bud1	NULL	null mutant	respond to	NULL				mating pheromone	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_13_13084_s_298	15657049	A  bud1 null mutant is able to respond to mating pheromone and to form shmoos ( ,  ), suggesting that the defect in Ste5 recruitment is not linked to a defect in Cdc24 binding to Rsr1/Bud1.	bind
37976	2	8817	7	NULL	NULL	0	NULL	statement 1	NULL		form	NULL				shmoos	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_13_13084_s_298	15657049	A  bud1 null mutant is able to respond to mating pheromone and to form shmoos ( ,  ), suggesting that the defect in Ste5 recruitment is not linked to a defect in Cdc24 binding to Rsr1/Bud1.	bind
37977	3	8817	7	NULL	NULL	0	NULL	 Cdc24	NULL		bind	NULL				Rsr1/Bud1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_13_13084_s_298	15657049	A  bud1 null mutant is able to respond to mating pheromone and to form shmoos ( ,  ), suggesting that the defect in Ste5 recruitment is not linked to a defect in Cdc24 binding to Rsr1/Bud1.	bind
37978	4	8817	7	10	NULL	0	NULL	Ste5	NULL	defect in recruitment of	is not linked to	NULL				statement 3	NULL	defect in			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_13_13084_s_298	15657049	A  bud1 null mutant is able to respond to mating pheromone and to form shmoos ( ,  ), suggesting that the defect in Ste5 recruitment is not linked to a defect in Cdc24 binding to Rsr1/Bud1.	bind
29397	1	8818	6	13	NULL	NULL	NULL	lipoprotein lipase	GP		bind			carboxyl-terminal fragment		low density lipoprotein receptor-related protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevnutr_19_0_141_s_1074	10448520	A  carboxyl-terminal fragment of lipoprotein lipase binds to the low density lipoprotein  receptor-related protein and inhibits lipase-mediated uptake of lipoprotein in cells.	bind
29399	2	8818	6	13	NULL	NULL	NULL	lipoprotein	GP	uptake of	is mediated by					lipase	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevnutr_19_0_141_s_1074	10448520	A  carboxyl-terminal fragment of lipoprotein lipase binds to the low density lipoprotein  receptor-related protein and inhibits lipase-mediated uptake of lipoprotein in cells.	bind
29400	3	8818	6	13	NULL	NULL	NULL	statement 1	Process		inhibits					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevnutr_19_0_141_s_1074	10448520	A  carboxyl-terminal fragment of lipoprotein lipase binds to the low density lipoprotein  receptor-related protein and inhibits lipase-mediated uptake of lipoprotein in cells.	bind
37979	1	8818	7	NULL	NULL	0	NULL	lipoprotein lipase	NULL		binds to	NULL		carboxyl-terminal fragment		low density lipoprotein receptor-related protein	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevnutr_19_0_141_s_1074	10448520	A  carboxyl-terminal fragment of lipoprotein lipase binds to the low density lipoprotein  receptor-related protein and inhibits lipase-mediated uptake of lipoprotein in cells.	bind
37980	2	8818	7	NULL	NULL	0	NULL	lipase	NULL		mediates	NULL				lipoprotein	NULL	uptake of			NULL	cells	0	NULL	NULL	NULL	gw70_annurevnutr_19_0_141_s_1074	10448520	A  carboxyl-terminal fragment of lipoprotein lipase binds to the low density lipoprotein  receptor-related protein and inhibits lipase-mediated uptake of lipoprotein in cells.	bind
37981	3	8818	7	NULL	NULL	0	NULL	statement 1	NULL		inhibits	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevnutr_19_0_141_s_1074	10448520	A  carboxyl-terminal fragment of lipoprotein lipase binds to the low density lipoprotein  receptor-related protein and inhibits lipase-mediated uptake of lipoprotein in cells.	bind
47116	1	8819	6	13	NULL	NULL	NULL	MC2	GP		delay					allograft rejection	Process				NULL	animal model	NULL	NULL	NULL	NULL	abs-batch0517-0529_int-immunopharmacol_5_11_16039552_s_5	16039552	A  cationic peptide (MC2) derived from the heparin-binding sequence of mouse  IFN-gamma was previously shown by our laboratory to delay allograft rejection  in an animal model.	bind
47117	2	8819	6	13	NULL	NULL	NULL	MC2	GP		is a type of					cationic peptide	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_int-immunopharmacol_5_11_16039552_s_5	16039552	A  cationic peptide (MC2) derived from the heparin-binding sequence of mouse  IFN-gamma was previously shown by our laboratory to delay allograft rejection  in an animal model.	bind
47118	3	8819	6	13	NULL	NULL	NULL	MC2	GP		is derived from					IFN-gamma	GP	mouse	heparin binding sequence		NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_int-immunopharmacol_5_11_16039552_s_5	16039552	A  cationic peptide (MC2) derived from the heparin-binding sequence of mouse  IFN-gamma was previously shown by our laboratory to delay allograft rejection  in an animal model.	bind
37982	1	8819	7	NULL	NULL	0	NULL	MC2	NULL		delay	NULL				allograft rejection	NULL				NULL	animal model	0	NULL	NULL	NULL	abs-batch0517-0529_int-immunopharmacol_5_11_16039552_s_5	16039552	A  cationic peptide (MC2) derived from the heparin-binding sequence of mouse  IFN-gamma was previously shown by our laboratory to delay allograft rejection  in an animal model.	bind
37983	2	8819	7	NULL	NULL	0	NULL	MC2	NULL		is a type of	NULL				cationic peptide	NULL				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_int-immunopharmacol_5_11_16039552_s_5	16039552	A  cationic peptide (MC2) derived from the heparin-binding sequence of mouse  IFN-gamma was previously shown by our laboratory to delay allograft rejection  in an animal model.	bind
37984	3	8819	7	NULL	NULL	0	NULL	MC2	NULL		is derived from	NULL				IFN-gamma	NULL	mouse	heparin-binding sequence		NULL		0	NULL	NULL	NULL	abs-batch0517-0529_int-immunopharmacol_5_11_16039552_s_5	16039552	A  cationic peptide (MC2) derived from the heparin-binding sequence of mouse  IFN-gamma was previously shown by our laboratory to delay allograft rejection  in an animal model.	bind
29601	1	8823	6	13	NULL	NULL	NULL			rat	restricts				OC box -76 to -99	OC	GP	expression of			NULL	osteoblasts	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_9248_s_42	15456894	A  cis regulatory sequence conserved in the segment of the proximal promoter of all species, known as the OC box ( - 76 to  - 99 in rat), encompasses a core HD protein binding site (CAATTAGT) that restricts OC expression to osteoblasts ( ,  ).	bind
29602	2	8823	6	13	NULL	NULL	NULL				is a binding site for				CAATTAGT	core HD protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_9248_s_42	15456894	A  cis regulatory sequence conserved in the segment of the proximal promoter of all species, known as the OC box ( - 76 to  - 99 in rat), encompasses a core HD protein binding site (CAATTAGT) that restricts OC expression to osteoblasts ( ,  ).	bind
29603	3	8823	6	13	NULL	NULL	NULL			rat	encompasses				OC box -76 to -99	statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_9248_s_42	15456894	A  cis regulatory sequence conserved in the segment of the proximal promoter of all species, known as the OC box ( - 76 to  - 99 in rat), encompasses a core HD protein binding site (CAATTAGT) that restricts OC expression to osteoblasts ( ,  ).	bind
37986	1	8823	7	NULL	NULL	0	NULL		NULL	rat	restricts	NULL			OC box - 76 to - 99	OC	NULL	expression of			NULL	osteoblasts	NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_9248_s_42	15456894	A  cis regulatory sequence conserved in the segment of the proximal promoter of all species, known as the OC box ( - 76 to  - 99 in rat), encompasses a core HD protein binding site (CAATTAGT) that restricts OC expression to osteoblasts ( ,  ).	bind
37987	2	8823	7	10	NULL	0	NULL		NULL		is a binding site for	NULL			CAATTAGT	core HD protein	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_9248_s_42	15456894	A  cis regulatory sequence conserved in the segment of the proximal promoter of all species, known as the OC box ( - 76 to  - 99 in rat), encompasses a core HD protein binding site (CAATTAGT) that restricts OC expression to osteoblasts ( ,  ).	bind
37988	3	8823	7	NULL	NULL	0	NULL		NULL		is conserved in	NULL			cis regulatory sequence		NULL			proximal promoter	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_20_9248_s_42	15456894	A  cis regulatory sequence conserved in the segment of the proximal promoter of all species, known as the OC box ( - 76 to  - 99 in rat), encompasses a core HD protein binding site (CAATTAGT) that restricts OC expression to osteoblasts ( ,  ).	bind
46948	4	8823	7	10	NULL	0	NULL		NULL	rat	encompass	NULL			OC box -76 to -99	statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_20_9248_s_42	15456894	A  cis regulatory sequence conserved in the segment of the proximal promoter of all species, known as the OC box ( - 76 to  - 99 in rat), encompasses a core HD protein binding site (CAATTAGT) that restricts OC expression to osteoblasts ( ,  ).	bind
29402	1	8824	6	13	NULL	NULL	NULL	stat6	GP		bind					IL-4 gene	GP	downstream of 			NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_18_0_451_s_413	10837066	A  cis-element capable of Stat6 binding downstream of the IL-4 structural gene was proposed  to act as a subset-specific silencing element in Th1 cells ( 214).	bind
29403	2	8824	6	13	NULL	NULL	NULL	statement 1	Process		acts as a 									silencing element	NULL	Th1 cells	NULL	NULL	NULL	NULL	gw70_annurevimmunol_18_0_451_s_413	10837066	A  cis-element capable of Stat6 binding downstream of the IL-4 structural gene was proposed  to act as a subset-specific silencing element in Th1 cells ( 214).	bind
37989	1	8824	7	10	NULL	0	NULL	Stat6	NULL		bind	NULL				IL-4 gene	NULL	downstream of			NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_18_0_451_s_413	10837066	A  cis-element capable of Stat6 binding downstream of the IL-4 structural gene was proposed  to act as a subset-specific silencing element in Th1 cells ( 214).	bind
37990	2	8824	7	10	NULL	0	NULL	statement 1	NULL		acts as a	NULL					NULL	subset-specific		silencing element	NULL	Th1 cells	NULL	NULL	NULL	NULL	gw70_annurevimmunol_18_0_451_s_413	10837066	A  cis-element capable of Stat6 binding downstream of the IL-4 structural gene was proposed  to act as a subset-specific silencing element in Th1 cells ( 214).	bind
29405	1	8826	6	13	NULL	NULL	NULL	Replication Inhibitor	GP		bind					PCNA	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_99_2_155_s_188	10535734	A  Comparison of Replication Inhibitor Binding to PCNA and RB69 Sliding Clamp Interactions  with DNA Polymerase A comparison of pol-CT with a peptide derived from the  eukaryotic DNA replication inhibitor protein p21CIP1 (Gulbis et al., 1996   ).	bind
29406	2	8826	6	13	NULL	NULL	NULL	RB69 sliding clamp	GP		interacts with					DNA Polymerase	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_99_2_155_s_188	10535734	A  Comparison of Replication Inhibitor Binding to PCNA and RB69 Sliding Clamp Interactions  with DNA Polymerase A comparison of pol-CT with a peptide derived from the  eukaryotic DNA replication inhibitor protein p21CIP1 (Gulbis et al., 1996   ).	bind
46949	3	8826	6	13	NULL	NULL	NULL	p21CIP1	GP		is a type of					eukaryotic DNA replication inhibitor protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_99_2_155_s_188	10535734	A  Comparison of Replication Inhibitor Binding to PCNA and RB69 Sliding Clamp Interactions  with DNA Polymerase A comparison of pol-CT with a peptide derived from the  eukaryotic DNA replication inhibitor protein p21CIP1 (Gulbis et al., 1996   ).	bind
37994	1	8826	7	NULL	NULL	0	NULL	Replication Inhibitor	NULL		binds to	NULL				PCNA	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_99_2_155_s_188	10535734	A  Comparison of Replication Inhibitor Binding to PCNA and RB69 Sliding Clamp Interactions  with DNA Polymerase A comparison of pol-CT with a peptide derived from the  eukaryotic DNA replication inhibitor protein p21CIP1 (Gulbis et al., 1996   ).	bind
37995	2	8826	7	10	NULL	0	NULL	RB69 Sliding Clamp			interacts with					DNA polymerase					NULL		NULL	NULL	NULL	NULL	gw60_cell_99_2_155_s_188	10535734	A  Comparison of Replication Inhibitor Binding to PCNA and RB69 Sliding Clamp Interactions  with DNA Polymerase A comparison of pol-CT with a peptide derived from the  eukaryotic DNA replication inhibitor protein p21CIP1 (Gulbis et al., 1996   ).	bind
37996	3	8826	7	NULL	NULL	0	NULL	p21CIP1	NULL		is a type of	NULL				eukaryotic DNA replication inhibitor protein	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_99_2_155_s_188	10535734	A  Comparison of Replication Inhibitor Binding to PCNA and RB69 Sliding Clamp Interactions  with DNA Polymerase A comparison of pol-CT with a peptide derived from the  eukaryotic DNA replication inhibitor protein p21CIP1 (Gulbis et al., 1996   ).	bind
29407	1	8827	6	13	NULL	NULL	NULL	CD28	GP		bind					B7	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-exp-med_181_4_7535334_s_8	7535334	A  comparison of the effects of mutations on the binding of CD28 and CTLA4  reveals that CD28 and CTLA4 binds to the same site on B7.	bind
29408	2	8827	6	13	NULL	NULL	NULL	CTLA4	GP		bind					B7	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-exp-med_181_4_7535334_s_8	7535334	A  comparison of the effects of mutations on the binding of CD28 and CTLA4  reveals that CD28 and CTLA4 binds to the same site on B7.	bind
37997	1	8827	7	NULL	NULL	0	NULL	 CD28	NULL		binds to	NULL				B7	NULL				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_j-exp-med_181_4_7535334_s_8	7535334	A  comparison of the effects of mutations on the binding of CD28 and CTLA4  reveals that CD28 and CTLA4 binds to the same site on B7.	bind
37998	2	8827	7	NULL	NULL	0	NULL	CTLA4 	NULL		binds to	NULL				B7	NULL				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_j-exp-med_181_4_7535334_s_8	7535334	A  comparison of the effects of mutations on the binding of CD28 and CTLA4  reveals that CD28 and CTLA4 binds to the same site on B7.	bind
37999	3	8827	7	NULL	NULL	0	NULL	statement 1	NULL	binding site of	is same as	NULL				statement 2	NULL	binding site of			NULL		0	NULL	NULL	NULL	abs-batch0680-0699_j-exp-med_181_4_7535334_s_8	7535334	A  comparison of the effects of mutations on the binding of CD28 and CTLA4  reveals that CD28 and CTLA4 binds to the same site on B7.	bind
29409	1	8831	6	13	NULL	NULL	NULL	t cell clone	Cell		does not bind					PIM/CD1d tetramers	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_29_10685_s_174	15243159	A  conventional T cell clone did not bind the PIM/CD1d tetramers ( Left).	bind
38015	1	8831	7	NULL	NULL	0	NULL	T cell clone	NULL		does not bind	NULL				PIM/CD1d tetramers	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_101_29_10685_s_174	15243159	A  conventional T cell clone did not bind the PIM/CD1d tetramers ( Left).	bind
29462	1	8832	6	13	NULL	NULL	NULL				bind				cre element	CcpA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_1_7_s_126	12486034	A  cre element, which could bind the CcpA carbon catabolite protein A, is located upstream of this multipromoter region.	bind
29463	2	8832	6	13	NULL	NULL	NULL	CcpA	GP		is					carbon catabolite protein A	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_1_7_s_126	12486034	A  cre element, which could bind the CcpA carbon catabolite protein A, is located upstream of this multipromoter region.	bind
46950	3	8832	6	13	NULL	NULL	NULL				is located				cre element	CcpA	GP	upstream of		multipromoter region	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_1_7_s_126	12486034	A  cre element, which could bind the CcpA carbon catabolite protein A, is located upstream of this multipromoter region.	bind
38016	1	8832	7	NULL	NULL	0	NULL		NULL		bind	NULL			cre element	CcpA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_185_1_7_s_126	12486034	A  cre element, which could bind the CcpA carbon catabolite protein A, is located upstream of this multipromoter region.	bind
38017	2	8832	7	NULL	NULL	0	NULL	CcpA	NULL		is	NULL				carbon catabolite protein A	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_185_1_7_s_126	12486034	A  cre element, which could bind the CcpA carbon catabolite protein A, is located upstream of this multipromoter region.	bind
38018	3	8832	7	10	NULL	0	NULL		NULL		is located	NULL			cre element	CcpA	NULL	upstream of		multipromoter region	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_1_7_s_126	12486034	A  cre element, which could bind the CcpA carbon catabolite protein A, is located upstream of this multipromoter region.	bind
29473	1	8838	6	13	NULL	NULL	NULL	C3bot	GP		bind					RalA-GTP	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_20_3670_s_261	16177825	A  direct consequence would be that C3bot binding to the RalA-GTP state is impaired  or at least largely reduced.	bind
38027	1	8838	7	NULL	NULL	0	NULL	C3bot	NULL		bind	NULL				RalA-GTP	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_24_20_3670_s_261	16177825	A  direct consequence would be that C3bot binding to the RalA-GTP state is impaired  or at least largely reduced.	bind
29474	1	8839	6	13	NULL	NULL	NULL	I-hs-APP	GP		bind					CBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_3_1613_s_134	8576160	A  dose-dependent inhibition of the binding of  I-hs-APP to  CBP by recombinant APP was observed in nanomolar concentrations ( B).	bind
29475	2	8839	6	13	NULL	NULL	NULL	APP	GP	recombinant	inhibits		dose dependently			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_3_1613_s_134	8576160	A  dose-dependent inhibition of the binding of  I-hs-APP to  CBP by recombinant APP was observed in nanomolar concentrations ( B).	bind
38028	1	8839	7	NULL	NULL	0	NULL	I-hs-APP	NULL		bind	NULL				CBP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_3_1613_s_134	8576160	A  dose-dependent inhibition of the binding of  I-hs-APP to  CBP by recombinant APP was observed in nanomolar concentrations ( B).	bind
38029	2	8839	7	10	NULL	0	NULL	APP	NULL	recombinant	inhibit	NULL	dose dependently			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_3_1613_s_134	8576160	A  dose-dependent inhibition of the binding of  I-hs-APP to  CBP by recombinant APP was observed in nanomolar concentrations ( B).	bind
29476	1	8841	6	13	NULL	NULL	NULL	rn-APP	GP	I-labeled	bind		saturably;;specifically			fibrillar collagen type I	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_3_1613_s_91	8576160	A  dot blot assay revealed that  I-labeled rn-APP binding to  fibrillar collagen type I and basement membrane collagen type IV ( 38) was saturable and specific.	bind
29477	2	8841	6	13	NULL	NULL	NULL	rn-APP	GP	I-labeled	bind		saturably;;specifically			basement membrane collagen type IV	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_3_1613_s_91	8576160	A  dot blot assay revealed that  I-labeled rn-APP binding to  fibrillar collagen type I and basement membrane collagen type IV ( 38) was saturable and specific.	bind
38031	1	8841	7	NULL	NULL	0	NULL	 rn-APP	NULL	I-labeled	bind	NULL	saturably;;specific			fibrillar collagen type I 	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_3_1613_s_91	8576160	A  dot blot assay revealed that  I-labeled rn-APP binding to  fibrillar collagen type I and basement membrane collagen type IV ( 38) was saturable and specific.	bind
38032	2	8841	7	NULL	NULL	0	NULL	 rn-APP	NULL	I-labeled 	bind	NULL	saturably;;specific			basement membrane collagen type IV	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_3_1613_s_91	8576160	A  dot blot assay revealed that  I-labeled rn-APP binding to  fibrillar collagen type I and basement membrane collagen type IV ( 38) was saturable and specific.	bind
46951	1	8842	6	13	NULL	NULL	NULL	BLMA	GP		bind					Bm molecules	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2311_s_231	11706014	A  dotted curve is drawn by assuming that the binding affinities of BLMA for two Bm molecules to the pockets are identical ( K d1 = 137.5 nM and  K d2 = 550 nM).	bind
38033	1	8842	7	NULL	NULL	0	NULL	BLMA	NULL		bind	NULL				Bm molecules	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_3_2311_s_231	11706014	A  dotted curve is drawn by assuming that the binding affinities of BLMA for two Bm molecules to the pockets are identical ( K d1 = 137.5 nM and  K d2 = 550 nM).	bind
29519	1	8843	6	13	NULL	NULL	NULL	GATA family member	GP	Drosophila	bind					Adh 	GP			regulatory sequences	NULL		NULL	NULL	NULL	NULL	gw60_insectbiochemmolbiol_31_6_679_s_228	11267906	A  Drosophila GATA family member that binds  Adh regulatory sequences is expressed in the developing fat body.	bind
29520	2	8843	6	13	NULL	NULL	NULL	GATA family member	GP	Drosophila	is expressed in					developing fat body	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_insectbiochemmolbiol_31_6_679_s_228	11267906	A  Drosophila GATA family member that binds  Adh regulatory sequences is expressed in the developing fat body.	bind
38034	1	8843	7	10	NULL	0	NULL	 GATA family member	NULL	Drosophila	binds	NULL				Adh	NULL			regulatory sequences	NULL		NULL	NULL	NULL	NULL	gw60_insectbiochemmolbiol_31_6_679_s_228	11267906	A  Drosophila GATA family member that binds  Adh regulatory sequences is expressed in the developing fat body.	bind
38035	2	8843	7	NULL	NULL	0	NULL	GATA family member	NULL	Drosophila	is expressed in	NULL				developing fat body	NULL				NULL		0	NULL	NULL	NULL	gw60_insectbiochemmolbiol_31_6_679_s_228	11267906	A  Drosophila GATA family member that binds  Adh regulatory sequences is expressed in the developing fat body.	bind
29521	1	8847	6	13	NULL	NULL	NULL	par-1	GP	Drosophila melanogaster 	plays a role in					embryonic-axis 	OrganismPart	formation of			NULL		NULL	NULL	NULL	NULL	gw60_development_130_17_4201_s_697	12874138	A  Drosophila melanogaster homologue of  Caenorhabditis elegans par-1 acts at an early step in embryonic-axis formation.	bind
29522	2	8847	6	13	NULL	NULL	NULL	par-1	GP	Drosophila melanogaster	is homologous to					par-1	GP	Caenorhabditis elegans			NULL		NULL	NULL	NULL	NULL	gw60_development_130_17_4201_s_697	12874138	A  Drosophila melanogaster homologue of  Caenorhabditis elegans par-1 acts at an early step in embryonic-axis formation.	bind
38176	1	8847	7	10	NULL	0	NULL	par-1	NULL	Drosophila melanogaster	plays a role in	NULL				embryonic axis	NULL	formation of			NULL		NULL	NULL	NULL	NULL	gw60_development_130_17_4201_s_697	12874138	A  Drosophila melanogaster homologue of  Caenorhabditis elegans par-1 acts at an early step in embryonic-axis formation.	bind
38177	2	8847	7	NULL	NULL	0	NULL	par-1	NULL	Caenorhabditis elegans	is homologous to	NULL				par-1	NULL	Drosophila melanogaster			NULL		0	NULL	NULL	NULL	gw60_development_130_17_4201_s_697	12874138	A  Drosophila melanogaster homologue of  Caenorhabditis elegans par-1 acts at an early step in embryonic-axis formation.	bind
29523	1	8848	6	13	NULL	NULL	NULL	TRAF	GP		is					TNF-receptor-associated factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_149_2_471_s_709	10769037	A  Drosophila TNF-receptor-associated factor (TRAF) binds the ste20 kinase Misshapen and activates Jun kinase.	bind
29524	2	8848	6	13	NULL	NULL	NULL	Misshapen	GP		is a type of					ste20 kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_149_2_471_s_709	10769037	A  Drosophila TNF-receptor-associated factor (TRAF) binds the ste20 kinase Misshapen and activates Jun kinase.	bind
29525	3	8848	6	13	NULL	NULL	NULL	TRAF	GP	drosophila	bind					misshapen	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_149_2_471_s_709	10769037	A  Drosophila TNF-receptor-associated factor (TRAF) binds the ste20 kinase Misshapen and activates Jun kinase.	bind
29526	4	8848	6	13	NULL	NULL	NULL	statement 1	GP		activates					jun kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_149_2_471_s_709	10769037	A  Drosophila TNF-receptor-associated factor (TRAF) binds the ste20 kinase Misshapen and activates Jun kinase.	bind
38178	1	8848	7	10	NULL	0	NULL	TRAF	NULL	Drosophila	binds 	NULL				Misshapen	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_149_2_471_s_709	10769037	A  Drosophila TNF-receptor-associated factor (TRAF) binds the ste20 kinase Misshapen and activates Jun kinase.	bind
38179	2	8848	7	NULL	NULL	0	NULL	statement 1	NULL		activates	NULL				Jun kinase	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_149_2_471_s_709	10769037	A  Drosophila TNF-receptor-associated factor (TRAF) binds the ste20 kinase Misshapen and activates Jun kinase.	bind
38180	3	8848	7	NULL	NULL	0	NULL	TRAF	NULL		is	NULL				TNF-receptor-associated factor	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_149_2_471_s_709	10769037	A  Drosophila TNF-receptor-associated factor (TRAF) binds the ste20 kinase Misshapen and activates Jun kinase.	bind
46952	4	8848	7	10	NULL	0	NULL	Misshapen	NULL		is a type of	NULL				ste20 kinase	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_149_2_471_s_709	10769037	A  Drosophila TNF-receptor-associated factor (TRAF) binds the ste20 kinase Misshapen and activates Jun kinase.	bind
29527	1	8849	6	13	NULL	NULL	NULL	dSlo clone	GP		bind		high affinity			CTX	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_1_11_s_249	10665815	A  dSlo clone that binds CTX with high affinity would be a valuable tool in future studies of these channels.	bind
38181	1	8849	7	NULL	NULL	0	NULL	dSlo clone	NULL		binds	NULL	high affinity			CTX	NULL				NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_39_1_11_s_249	10665815	A  dSlo clone that binds CTX with high affinity would be a valuable tool in future studies of these channels.	bind
29528	1	8850	6	13	NULL	NULL	NULL	VDR/RXR heterodimer	GP		bind					TRPV6 gene	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_mol-endocrinol_20_6_16574738_s_11	16574738	A  final ChIP assay revealed that VDR/RXR heterodimer binding to the TRPV6  gene was accompanied by both the recruitment of steroid receptor coactivator  1 as well as a broad change in histone 4 acetylation.	bind
29529	2	8850	6	13	NULL	NULL	NULL	statement 1	Process		is accompanied by					steroid receptor coactivator 1	GP	recruitment of			NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_mol-endocrinol_20_6_16574738_s_11	16574738	A  final ChIP assay revealed that VDR/RXR heterodimer binding to the TRPV6  gene was accompanied by both the recruitment of steroid receptor coactivator  1 as well as a broad change in histone 4 acetylation.	bind
29530	3	8850	6	13	NULL	NULL	NULL	statement 1	Process		is accompanied by					histone 4	GP	change in acetylation of 			NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_mol-endocrinol_20_6_16574738_s_11	16574738	A  final ChIP assay revealed that VDR/RXR heterodimer binding to the TRPV6  gene was accompanied by both the recruitment of steroid receptor coactivator  1 as well as a broad change in histone 4 acetylation.	bind
38182	1	8850	7	NULL	NULL	0	NULL	VDR/RXR heterodimer	NULL		bind	NULL				TRPV6 gene	NULL				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_mol-endocrinol_20_6_16574738_s_11	16574738	A  final ChIP assay revealed that VDR/RXR heterodimer binding to the TRPV6  gene was accompanied by both the recruitment of steroid receptor coactivator  1 as well as a broad change in histone 4 acetylation.	bind
38183	2	8850	7	10	NULL	0	NULL	statement 1	NULL		is accompanied by	NULL				steroid receptor coactivator 1	NULL	recruitment of			NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_mol-endocrinol_20_6_16574738_s_11	16574738	A  final ChIP assay revealed that VDR/RXR heterodimer binding to the TRPV6  gene was accompanied by both the recruitment of steroid receptor coactivator  1 as well as a broad change in histone 4 acetylation.	bind
38184	3	8850	7	10	NULL	0	NULL	statement 1	NULL		is accompanied by	NULL				histone 4	NULL	change in acetylation of			NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_mol-endocrinol_20_6_16574738_s_11	16574738	A  final ChIP assay revealed that VDR/RXR heterodimer binding to the TRPV6  gene was accompanied by both the recruitment of steroid receptor coactivator  1 as well as a broad change in histone 4 acetylation.	bind
29531	1	8851	6	13	NULL	NULL	NULL	agrin	GP		bind					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_85_4_513_s_28	8653787	A  four amino acid insertion at the Y position causes a modest additional  increase in the activity of agrins having an insertion at the Z  position, and the Y insertion also seems to be involved in the binding  of agrin to heparin and proteoglycans (Ferns et al., 1993   ;  Hoch  et al., 1994   ).	bind
29532	2	8851	6	13	NULL	NULL	NULL	agrin	GP		bind					proteoglycans	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_85_4_513_s_28	8653787	A  four amino acid insertion at the Y position causes a modest additional  increase in the activity of agrins having an insertion at the Z  position, and the Y insertion also seems to be involved in the binding  of agrin to heparin and proteoglycans (Ferns et al., 1993   ;  Hoch  et al., 1994   ).	bind
29533	3	8851	6	13	NULL	NULL	NULL	four amino acid	AminoAcid		inserted at					Y position	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_85_4_513_s_28	8653787	A  four amino acid insertion at the Y position causes a modest additional  increase in the activity of agrins having an insertion at the Z  position, and the Y insertion also seems to be involved in the binding  of agrin to heparin and proteoglycans (Ferns et al., 1993   ;  Hoch  et al., 1994   ).	bind
29534	4	8851	6	13	NULL	NULL	NULL	statement 3	Process		is involved in					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_85_4_513_s_28	8653787	A  four amino acid insertion at the Y position causes a modest additional  increase in the activity of agrins having an insertion at the Z  position, and the Y insertion also seems to be involved in the binding  of agrin to heparin and proteoglycans (Ferns et al., 1993   ;  Hoch  et al., 1994   ).	bind
29535	5	8851	6	13	NULL	NULL	NULL	statement 3	Process		is involved in					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_85_4_513_s_28	8653787	A  four amino acid insertion at the Y position causes a modest additional  increase in the activity of agrins having an insertion at the Z  position, and the Y insertion also seems to be involved in the binding  of agrin to heparin and proteoglycans (Ferns et al., 1993   ;  Hoch  et al., 1994   ).	bind
29536	6	8851	6	13	NULL	NULL	NULL	agrins	GP		have insertion at					Z postition	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_85_4_513_s_28	8653787	A  four amino acid insertion at the Y position causes a modest additional  increase in the activity of agrins having an insertion at the Z  position, and the Y insertion also seems to be involved in the binding  of agrin to heparin and proteoglycans (Ferns et al., 1993   ;  Hoch  et al., 1994   ).	bind
29537	7	8851	6	13	NULL	NULL	NULL	statement 3	Process		increases		modestly			statement 6	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_cell_85_4_513_s_28	8653787	A  four amino acid insertion at the Y position causes a modest additional  increase in the activity of agrins having an insertion at the Z  position, and the Y insertion also seems to be involved in the binding  of agrin to heparin and proteoglycans (Ferns et al., 1993   ;  Hoch  et al., 1994   ).	bind
38185	1	8851	7	NULL	NULL	0	NULL	agrin	NULL		bind	NULL				heparin	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_85_4_513_s_28	8653787	A  four amino acid insertion at the Y position causes a modest additional  increase in the activity of agrins having an insertion at the Z  position, and the Y insertion also seems to be involved in the binding  of agrin to heparin and proteoglycans (Ferns et al., 1993   ;  Hoch  et al., 1994   ).	bind
38186	2	8851	7	NULL	NULL	0	NULL	agrin	NULL		bind	NULL				proteoglycans	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_85_4_513_s_28	8653787	A  four amino acid insertion at the Y position causes a modest additional  increase in the activity of agrins having an insertion at the Z  position, and the Y insertion also seems to be involved in the binding  of agrin to heparin and proteoglycans (Ferns et al., 1993   ;  Hoch  et al., 1994   ).	bind
29538	1	8852	6	13	NULL	NULL	NULL	lectin	GP	Gal-specific	bind					asialyl-tetraantennary N-linked oligosaccharide	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_41_24024_s_23	7592600	A  Gal-specific lectin that binds asialyl-tetraantennary  N-linked  oligosaccharides and a Fuc/GlcNAc binding lectin have been found on rat  alveolar macrophages and Kupffer cells( 17,  18) .	bind
29539	2	8852	6	13	NULL	NULL	NULL	lectin	GP	Gal-specific	is found on					alveolar macrophages	Cell	rat			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_41_24024_s_23	7592600	A  Gal-specific lectin that binds asialyl-tetraantennary  N-linked  oligosaccharides and a Fuc/GlcNAc binding lectin have been found on rat  alveolar macrophages and Kupffer cells( 17,  18) .	bind
29540	3	8852	6	13	NULL	NULL	NULL	lectin	GP	Gal-specific	is found on					Kupffer cells	Cell	rat			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_41_24024_s_23	7592600	A  Gal-specific lectin that binds asialyl-tetraantennary  N-linked  oligosaccharides and a Fuc/GlcNAc binding lectin have been found on rat  alveolar macrophages and Kupffer cells( 17,  18) .	bind
29541	4	8852	6	13	NULL	NULL	NULL	lectin	GP		bind					Fuc/GlcNAc	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_41_24024_s_23	7592600	A  Gal-specific lectin that binds asialyl-tetraantennary  N-linked  oligosaccharides and a Fuc/GlcNAc binding lectin have been found on rat  alveolar macrophages and Kupffer cells( 17,  18) .	bind
29542	5	8852	6	13	NULL	NULL	NULL	lectin	GP		is found on					alveolar macrophages	Cell	rat			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_41_24024_s_23	7592600	A  Gal-specific lectin that binds asialyl-tetraantennary  N-linked  oligosaccharides and a Fuc/GlcNAc binding lectin have been found on rat  alveolar macrophages and Kupffer cells( 17,  18) .	bind
29543	6	8852	6	13	NULL	NULL	NULL	lectin	GP		is found on					Kupffer cells	Cell	rat			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_41_24024_s_23	7592600	A  Gal-specific lectin that binds asialyl-tetraantennary  N-linked  oligosaccharides and a Fuc/GlcNAc binding lectin have been found on rat  alveolar macrophages and Kupffer cells( 17,  18) .	bind
38190	1	8852	7	10	NULL	0	NULL	lectin	NULL	Gal-specific	bind	NULL				asialyl-tetraantennary N-linked oligosaccharides	NULL				NULL	rat alveolar macrophages	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_41_24024_s_23	7592600	A  Gal-specific lectin that binds asialyl-tetraantennary  N-linked  oligosaccharides and a Fuc/GlcNAc binding lectin have been found on rat  alveolar macrophages and Kupffer cells( 17,  18) .	bind
38191	2	8852	7	10	NULL	0	NULL	lectin	NULL	Gal-specific	bind	NULL				asialyl-tetraantennary N-linked oligosaccharides	NULL				NULL	rat Kupffer cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_41_24024_s_23	7592600	A  Gal-specific lectin that binds asialyl-tetraantennary  N-linked  oligosaccharides and a Fuc/GlcNAc binding lectin have been found on rat  alveolar macrophages and Kupffer cells( 17,  18) .	bind
38192	3	8852	7	NULL	NULL	0	NULL	Fuc/GlcNAc	NULL		bind	NULL				lectin	NULL				NULL	rat alveolar macrophages	0	NULL	NULL	NULL	gw60_jbiolchem_270_41_24024_s_23	7592600	A  Gal-specific lectin that binds asialyl-tetraantennary  N-linked  oligosaccharides and a Fuc/GlcNAc binding lectin have been found on rat  alveolar macrophages and Kupffer cells( 17,  18) .	bind
38194	4	8852	7	NULL	NULL	0	NULL	Fuc/GlcNAc	NULL		bind	NULL				lectin	NULL				NULL	rat Kupffer cells	0	NULL	NULL	NULL	gw60_jbiolchem_270_41_24024_s_23	7592600	A  Gal-specific lectin that binds asialyl-tetraantennary  N-linked  oligosaccharides and a Fuc/GlcNAc binding lectin have been found on rat  alveolar macrophages and Kupffer cells( 17,  18) .	bind
29544	2	8853	6	13	NULL	NULL	NULL	statement 1	GP		bind			amino terminal half		F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_32331_s_146	10915794	A  GST  fusion protein containing the amino-terminal half of B1 binds  F-actin.	bind
56165	1	8853	6	13	NULL	NULL	NULL	GST fusion protein	GP		contains					B1	GP		amino-terminal half		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_32331_s_146	10915794	A  GST  fusion protein containing the amino-terminal half of B1 binds  F-actin.	bind
38201	2	8853	7	NULL	NULL	0	NULL	statement 1	NULL		binds	NULL				F-actin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_32331_s_146	10915794	A  GST  fusion protein containing the amino-terminal half of B1 binds  F-actin.	bind
38203	1	8853	7	10	NULL	0	NULL	GST fusion protein			contains					B1			amino-terminal half		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_32331_s_146	10915794	A  GST  fusion protein containing the amino-terminal half of B1 binds  F-actin.	bind
29547	1	8855	6	13	NULL	NULL	NULL	JNK antisense oligonucleotide	NucleicAcid		downregulates					AP-1	GP	binding activity of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_24_21618_s_274	11290748	A  JNK  antisense oligonucleotide down-regulates the binding activity of AP-1 and NF-kappaB.	bind
29548	2	8855	6	13	NULL	NULL	NULL	JNK antisense oligonucleotide	NucleicAcid		downregulates					NF-kappaB	GP	binding activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_24_21618_s_274	11290748	A  JNK  antisense oligonucleotide down-regulates the binding activity of AP-1 and NF-kappaB.	bind
38211	1	8855	7	NULL	NULL	0	NULL	JNK antisense oligonucleotide	NULL		downregulates	NULL				AP-1	NULL	binding activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_24_21618_s_274	11290748	A  JNK  antisense oligonucleotide down-regulates the binding activity of AP-1 and NF-kappaB.	bind
38212	2	8855	7	NULL	NULL	0	NULL	JNK antisense oligonucleotide	NULL		downregulates	NULL				NF-kappaB	NULL	binding activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_24_21618_s_274	11290748	A  JNK  antisense oligonucleotide down-regulates the binding activity of AP-1 and NF-kappaB.	bind
47530	1	8856	6	13	NULL	NULL	NULL	FAD	Chemical		bind		specifically			apo-PchF	GP		flavin binding site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31202_s_212	8537385	A  K   value of 15 muM  at 25  degrees C and pH  7.0 was determined by fluorescence quenching of bound FAD; however, the  maximum fluorescence quenching was about 4 times greaterR than expected  if specific binding of FAD to the flavin binding site apo-PchF   had caused complete quenching of the FAD fluorescence.	bind
38215	1	8856	7	NULL	NULL	0	NULL	FAD 	NULL		bind	NULL	specifically			apo-PchF	NULL		flavin binding site 		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31202_s_212	8537385	A  K   value of 15 muM  at 25  degrees C and pH  7.0 was determined by fluorescence quenching of bound FAD; however, the  maximum fluorescence quenching was about 4 times greaterR than expected  if specific binding of FAD to the flavin binding site apo-PchF   had caused complete quenching of the FAD fluorescence.	bind
29549	1	8857	6	13	NULL	NULL	NULL	receptor	GP	mutant 	does not bind			N250A		[125]I-AB-MECA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_21_19056_s_127	11891221	A  K i value could not be determined (ND) for the N250A (6.55) mutant receptor, as this mutant receptor did bind to the agonist radioligand [125]I-AB-MECA or the antagonist radioligand [3]PSB-11.	bind
29550	2	8857	6	13	NULL	NULL	NULL	[125]I-AB-MECA	Chemical		is a type of					agonist radioligand	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_21_19056_s_127	11891221	A  K i value could not be determined (ND) for the N250A (6.55) mutant receptor, as this mutant receptor did bind to the agonist radioligand [125]I-AB-MECA or the antagonist radioligand [3]PSB-11.	bind
29551	3	8857	6	13	NULL	NULL	NULL	receptor	GP	mutant	does not bind			N250A		PSB-11	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_21_19056_s_127	11891221	A  K i value could not be determined (ND) for the N250A (6.55) mutant receptor, as this mutant receptor did bind to the agonist radioligand [125]I-AB-MECA or the antagonist radioligand [3]PSB-11.	bind
29552	4	8857	6	13	NULL	NULL	NULL	PSB-11	Chemical		is a type of					antagonist radioligand	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_21_19056_s_127	11891221	A  K i value could not be determined (ND) for the N250A (6.55) mutant receptor, as this mutant receptor did bind to the agonist radioligand [125]I-AB-MECA or the antagonist radioligand [3]PSB-11.	bind
38222	1	8857	7	10	NULL	0	NULL	receptor	NULL	mutant	does not bind	NULL		 N250A		[125]I-AB-MECA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_21_19056_s_127	11891221	A  K i value could not be determined (ND) for the N250A (6.55) mutant receptor, as this mutant receptor did bind to the agonist radioligand [125]I-AB-MECA or the antagonist radioligand [3]PSB-11.	bind
38223	2	8857	7	10	NULL	0	NULL	receptor	NULL	mutant	does not bind	NULL		N250A		[3]PSB-11	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_21_19056_s_127	11891221	A  K i value could not be determined (ND) for the N250A (6.55) mutant receptor, as this mutant receptor did bind to the agonist radioligand [125]I-AB-MECA or the antagonist radioligand [3]PSB-11.	bind
46953	3	8857	7	10	NULL	0	NULL	[125]I-AB-MECA	NULL		is a type of	NULL				agonist radioligand	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_21_19056_s_127	11891221	A  K i value could not be determined (ND) for the N250A (6.55) mutant receptor, as this mutant receptor did bind to the agonist radioligand [125]I-AB-MECA or the antagonist radioligand [3]PSB-11.	bind
46955	4	8857	7	10	NULL	0	NULL	[3]PSB-11	NULL		is a type of	NULL				antagonist radioligand 	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_21_19056_s_127	11891221	A  K i value could not be determined (ND) for the N250A (6.55) mutant receptor, as this mutant receptor did bind to the agonist radioligand [125]I-AB-MECA or the antagonist radioligand [3]PSB-11.	bind
29553	1	8858	6	13	NULL	NULL	NULL	CcpA	GP		bind					phoPR	GP			cre site	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_4_1266_s_278	16452408	A  Kd of  0.5 nM was calculated for CcpA binding to the  phoPR cre site from the footprint data (data not shown) using the procedure described by Kim et. al ( ).	bind
38224	1	8858	7	NULL	NULL	0	NULL	 CcpA	NULL		bind	NULL				 phoPR	NULL			cre site	NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_4_1266_s_278	16452408	A  Kd of  0.5 nM was calculated for CcpA binding to the  phoPR cre site from the footprint data (data not shown) using the procedure described by Kim et. al ( ).	bind
29554	1	8860	6	13	NULL	NULL	NULL	dibucaine	Chemical		bind					spectrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_532_3_396_s_82	12482599	A  Kd of 35  M was estimated for dibucaine binding to spectrin and was independent of ionic strength of the buffer, in the presence of both low and high concentrations of NaCl ( Table 1).	bind
38225	1	8860	7	NULL	NULL	0	NULL	dibucaine	NULL		bind	NULL				spectrin	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_532_3_396_s_82	12482599	A  Kd of 35  M was estimated for dibucaine binding to spectrin and was independent of ionic strength of the buffer, in the presence of both low and high concentrations of NaCl ( Table 1).	bind
29555	1	8861	6	13	NULL	NULL	NULL	ferrocyanide	Chemical		bind					SOR	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_40_14750_s_51	17001016	A  Kd value of 0.80  plus-or-minus  0.07 muM was determined for the binding of ferrocyanide to SOR (Fig. 6, which is published as  supporting information on the PNAS web site).	bind
38228	1	8861	7	NULL	NULL	0	NULL	ferrocyanide	NULL		bind	NULL				SOR	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_103_40_14750_s_51	17001016	A  Kd value of 0.80  plus-or-minus  0.07 muM was determined for the binding of ferrocyanide to SOR (Fig. 6, which is published as  supporting information on the PNAS web site).	bind
29556	1	8862	6	13	NULL	NULL	NULL	CPX	GP		bind					CHO-hA1AdoR membrane	GP				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_298_1_209_s_145	11408544	A  Kd value of 1 nM for [3]CPX binding to CHO-hA1AdoR membrane was used in calculation of  Ki values.	bind
38229	1	8862	7	NULL	NULL	0	NULL	[3]CPX	NULL		bind	NULL				CHO-hA1AdoR membrane	NULL				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_298_1_209_s_145	11408544	A  Kd value of 1 nM for [3]CPX binding to CHO-hA1AdoR membrane was used in calculation of  Ki values.	bind
29557	1	8863	6	13	NULL	NULL	NULL	MPT	GP		bind					XdhC	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_23_15701_s_149	16597619	A  KD value of 3.6  plus-or-minus  0.1 muM was obtained for Moco binding, and a  KD value of 3.5  plus-or-minus  0.3 muM was obtained for MPT binding to XdhC at 4  degrees C, showing that XdhC is able to bind both molecules with the same efficiency in stoichiometric amounts.	bind
46956	2	8863	6	13	NULL	NULL	NULL	Moco	GP		bind					XdhC	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_23_15701_s_149	16597619	A  KD value of 3.6  plus-or-minus  0.1 muM was obtained for Moco binding, and a  KD value of 3.5  plus-or-minus  0.3 muM was obtained for MPT binding to XdhC at 4  degrees C, showing that XdhC is able to bind both molecules with the same efficiency in stoichiometric amounts.	bind
46957	3	8863	6	13	NULL	NULL	NULL	statement 1	Process		same efficiency as					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_23_15701_s_149	16597619	A  KD value of 3.6  plus-or-minus  0.1 muM was obtained for Moco binding, and a  KD value of 3.5  plus-or-minus  0.3 muM was obtained for MPT binding to XdhC at 4  degrees C, showing that XdhC is able to bind both molecules with the same efficiency in stoichiometric amounts.	bind
38230	1	8863	7	NULL	NULL	0	NULL	Moco	NULL		bind	NULL				XdhC	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_23_15701_s_149	16597619	A  KD value of 3.6  plus-or-minus  0.1 muM was obtained for Moco binding, and a  KD value of 3.5  plus-or-minus  0.3 muM was obtained for MPT binding to XdhC at 4  degrees C, showing that XdhC is able to bind both molecules with the same efficiency in stoichiometric amounts.	bind
38231	2	8863	7	NULL	NULL	0	NULL	MPT	NULL		bind	NULL				XdhC	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_23_15701_s_149	16597619	A  KD value of 3.6  plus-or-minus  0.1 muM was obtained for Moco binding, and a  KD value of 3.5  plus-or-minus  0.3 muM was obtained for MPT binding to XdhC at 4  degrees C, showing that XdhC is able to bind both molecules with the same efficiency in stoichiometric amounts.	bind
38232	3	8863	7	NULL	NULL	0	NULL	statement 1	NULL		has same efficiency as	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_23_15701_s_149	16597619	A  KD value of 3.6  plus-or-minus  0.1 muM was obtained for Moco binding, and a  KD value of 3.5  plus-or-minus  0.3 muM was obtained for MPT binding to XdhC at 4  degrees C, showing that XdhC is able to bind both molecules with the same efficiency in stoichiometric amounts.	bind
29558	1	8864	6	13	NULL	NULL	NULL	pregnenolone 	Chemical		bind					sigma 1	GP				NULL	SH-SY5Y cells	NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_306_3_934_s_157	12750428	A  Ki value at sigma receptors in brain tissue has  not been reported, but we found that pregnenolone competed for  sigma1 binding with a  Ki value of 980   plus-or-minus  340 nM in SH-SY5Y cells (Werling,  2002  ).	bind
38233	1	8864	7	NULL	NULL	0	NULL	pregnenolone	NULL		bind	NULL				sigma1	NULL				NULL	SH-SY5Y cells	0	NULL	NULL	NULL	gw60_jpharmacolexpther_306_3_934_s_157	12750428	A  Ki value at sigma receptors in brain tissue has  not been reported, but we found that pregnenolone competed for  sigma1 binding with a  Ki value of 980   plus-or-minus  340 nM in SH-SY5Y cells (Werling,  2002  ).	bind
29559	1	8867	6	13	NULL	NULL	NULL	RA	Chemical		bind					RAR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20258_s_166	7657595	A  ligand-induced three-dimensional conformation may occur upon binding of  RA to an RAR such that the ligand binding domain ```folds'''   around the ligand leaving lysine 220 and arginine 269 to interact with  the carboxylate tail and methionine 406 and, possibly, isoleucine 410,  to interact with the methyl group located at the 9 position on  9- cis-RA.	bind
50886	2	8867	6	13	NULL	NULL	NULL	statement 1	Process		folds around			ligand binding domain		ligand	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20258_s_166	7657595	A  ligand-induced three-dimensional conformation may occur upon binding of  RA to an RAR such that the ligand binding domain ```folds'''   around the ligand leaving lysine 220 and arginine 269 to interact with  the carboxylate tail and methionine 406 and, possibly, isoleucine 410,  to interact with the methyl group located at the 9 position on  9- cis-RA.	bind
50887	3	8867	6	13	NULL	NULL	NULL	RAR	GP		interacts with			lysine 220		RAR	GP		carboxylate tail		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20258_s_166	7657595	A  ligand-induced three-dimensional conformation may occur upon binding of  RA to an RAR such that the ligand binding domain ```folds'''   around the ligand leaving lysine 220 and arginine 269 to interact with  the carboxylate tail and methionine 406 and, possibly, isoleucine 410,  to interact with the methyl group located at the 9 position on  9- cis-RA.	bind
50888	4	8867	6	13	NULL	NULL	NULL	RAR	GP		interacts with			arginine 269		RAR	GP		carboxylate tail		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20258_s_166	7657595	A  ligand-induced three-dimensional conformation may occur upon binding of  RA to an RAR such that the ligand binding domain ```folds'''   around the ligand leaving lysine 220 and arginine 269 to interact with  the carboxylate tail and methionine 406 and, possibly, isoleucine 410,  to interact with the methyl group located at the 9 position on  9- cis-RA.	bind
50889	5	8867	6	13	NULL	NULL	NULL	RAR	GP		interacts with			lysine 220		RAR	GP		methionine 406		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20258_s_166	7657595	A  ligand-induced three-dimensional conformation may occur upon binding of  RA to an RAR such that the ligand binding domain ```folds'''   around the ligand leaving lysine 220 and arginine 269 to interact with  the carboxylate tail and methionine 406 and, possibly, isoleucine 410,  to interact with the methyl group located at the 9 position on  9- cis-RA.	bind
50890	6	8867	6	13	NULL	NULL	NULL	RAR	GP		interacts with			arginine 269		RAR	GP		methionine 406		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20258_s_166	7657595	A  ligand-induced three-dimensional conformation may occur upon binding of  RA to an RAR such that the ligand binding domain ```folds'''   around the ligand leaving lysine 220 and arginine 269 to interact with  the carboxylate tail and methionine 406 and, possibly, isoleucine 410,  to interact with the methyl group located at the 9 position on  9- cis-RA.	bind
50891	7	8867	6	13	NULL	NULL	NULL	RAR	GP		interacts with			isoleucine 410		9-cis RA	Chemical		methyl group located at the 9 position		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20258_s_166	7657595	A  ligand-induced three-dimensional conformation may occur upon binding of  RA to an RAR such that the ligand binding domain ```folds'''   around the ligand leaving lysine 220 and arginine 269 to interact with  the carboxylate tail and methionine 406 and, possibly, isoleucine 410,  to interact with the methyl group located at the 9 position on  9- cis-RA.	bind
50892	8	8867	6	13	NULL	NULL	NULL	statement 2	Process		allows					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20258_s_166	7657595	A  ligand-induced three-dimensional conformation may occur upon binding of  RA to an RAR such that the ligand binding domain ```folds'''   around the ligand leaving lysine 220 and arginine 269 to interact with  the carboxylate tail and methionine 406 and, possibly, isoleucine 410,  to interact with the methyl group located at the 9 position on  9- cis-RA.	bind
50893	9	8867	6	13	NULL	NULL	NULL	statement 2	Process		allows					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20258_s_166	7657595	A  ligand-induced three-dimensional conformation may occur upon binding of  RA to an RAR such that the ligand binding domain ```folds'''   around the ligand leaving lysine 220 and arginine 269 to interact with  the carboxylate tail and methionine 406 and, possibly, isoleucine 410,  to interact with the methyl group located at the 9 position on  9- cis-RA.	bind
50894	10	8867	6	13	NULL	NULL	NULL	statement 2	Process		allows					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20258_s_166	7657595	A  ligand-induced three-dimensional conformation may occur upon binding of  RA to an RAR such that the ligand binding domain ```folds'''   around the ligand leaving lysine 220 and arginine 269 to interact with  the carboxylate tail and methionine 406 and, possibly, isoleucine 410,  to interact with the methyl group located at the 9 position on  9- cis-RA.	bind
50895	11	8867	6	13	NULL	NULL	NULL	statement 2	Process		allows					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20258_s_166	7657595	A  ligand-induced three-dimensional conformation may occur upon binding of  RA to an RAR such that the ligand binding domain ```folds'''   around the ligand leaving lysine 220 and arginine 269 to interact with  the carboxylate tail and methionine 406 and, possibly, isoleucine 410,  to interact with the methyl group located at the 9 position on  9- cis-RA.	bind
50896	12	8867	6	13	NULL	NULL	NULL	statement 2	Process		allows					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20258_s_166	7657595	A  ligand-induced three-dimensional conformation may occur upon binding of  RA to an RAR such that the ligand binding domain ```folds'''   around the ligand leaving lysine 220 and arginine 269 to interact with  the carboxylate tail and methionine 406 and, possibly, isoleucine 410,  to interact with the methyl group located at the 9 position on  9- cis-RA.	bind
38244	1	8867	7	NULL	NULL	0	NULL	RA	NULL		bind	NULL				RAR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20258_s_166	7657595	A  ligand-induced three-dimensional conformation may occur upon binding of  RA to an RAR such that the ligand binding domain ```folds'''   around the ligand leaving lysine 220 and arginine 269 to interact with  the carboxylate tail and methionine 406 and, possibly, isoleucine 410,  to interact with the methyl group located at the 9 position on  9- cis-RA.	bind
38247	2	8867	7	NULL	NULL	0	NULL	statement 1	NULL		folds around	NULL		ligand binding domain		ligand	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20258_s_166	7657595	A  ligand-induced three-dimensional conformation may occur upon binding of  RA to an RAR such that the ligand binding domain ```folds'''   around the ligand leaving lysine 220 and arginine 269 to interact with  the carboxylate tail and methionine 406 and, possibly, isoleucine 410,  to interact with the methyl group located at the 9 position on  9- cis-RA.	bind
38250	3	8867	7	NULL	NULL	0	NULL	RAR	NULL		interacts with	NULL		lysine 220 		RAR	NULL		carboxylate tail		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20258_s_166	7657595	A  ligand-induced three-dimensional conformation may occur upon binding of  RA to an RAR such that the ligand binding domain ```folds'''   around the ligand leaving lysine 220 and arginine 269 to interact with  the carboxylate tail and methionine 406 and, possibly, isoleucine 410,  to interact with the methyl group located at the 9 position on  9- cis-RA.	bind
38251	4	8867	7	NULL	NULL	0	NULL	RAR	NULL		interacts with	NULL		arginine 269		RAR	NULL		carboxylate tail		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20258_s_166	7657595	A  ligand-induced three-dimensional conformation may occur upon binding of  RA to an RAR such that the ligand binding domain ```folds'''   around the ligand leaving lysine 220 and arginine 269 to interact with  the carboxylate tail and methionine 406 and, possibly, isoleucine 410,  to interact with the methyl group located at the 9 position on  9- cis-RA.	bind
38252	5	8867	7	NULL	NULL	0	NULL	RAR	NULL		interacts with	NULL		lysine 220 		RAR	NULL		 methionine 406		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20258_s_166	7657595	A  ligand-induced three-dimensional conformation may occur upon binding of  RA to an RAR such that the ligand binding domain ```folds'''   around the ligand leaving lysine 220 and arginine 269 to interact with  the carboxylate tail and methionine 406 and, possibly, isoleucine 410,  to interact with the methyl group located at the 9 position on  9- cis-RA.	bind
38253	6	8867	7	NULL	NULL	0	NULL	RAR	NULL		interacts with	NULL		arginine 269		RAR	NULL		 methionine 406		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20258_s_166	7657595	A  ligand-induced three-dimensional conformation may occur upon binding of  RA to an RAR such that the ligand binding domain ```folds'''   around the ligand leaving lysine 220 and arginine 269 to interact with  the carboxylate tail and methionine 406 and, possibly, isoleucine 410,  to interact with the methyl group located at the 9 position on  9- cis-RA.	bind
38254	7	8867	7	NULL	NULL	0	NULL	RAR	NULL		interacts with	NULL		isoleucine 410		 9- cis-RA	NULL		methyl group  at  9th position		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20258_s_166	7657595	A  ligand-induced three-dimensional conformation may occur upon binding of  RA to an RAR such that the ligand binding domain ```folds'''   around the ligand leaving lysine 220 and arginine 269 to interact with  the carboxylate tail and methionine 406 and, possibly, isoleucine 410,  to interact with the methyl group located at the 9 position on  9- cis-RA.	bind
38255	8	8867	7	NULL	NULL	0	NULL	statement 2	NULL		allows	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20258_s_166	7657595	A  ligand-induced three-dimensional conformation may occur upon binding of  RA to an RAR such that the ligand binding domain ```folds'''   around the ligand leaving lysine 220 and arginine 269 to interact with  the carboxylate tail and methionine 406 and, possibly, isoleucine 410,  to interact with the methyl group located at the 9 position on  9- cis-RA.	bind
50851	9	8867	7	NULL	NULL	0	NULL	statement 2	NULL		allows	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20258_s_166	7657595	A  ligand-induced three-dimensional conformation may occur upon binding of  RA to an RAR such that the ligand binding domain ```folds'''   around the ligand leaving lysine 220 and arginine 269 to interact with  the carboxylate tail and methionine 406 and, possibly, isoleucine 410,  to interact with the methyl group located at the 9 position on  9- cis-RA.	bind
50852	10	8867	7	NULL	NULL	0	NULL	statement 2	NULL		allows	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20258_s_166	7657595	A  ligand-induced three-dimensional conformation may occur upon binding of  RA to an RAR such that the ligand binding domain ```folds'''   around the ligand leaving lysine 220 and arginine 269 to interact with  the carboxylate tail and methionine 406 and, possibly, isoleucine 410,  to interact with the methyl group located at the 9 position on  9- cis-RA.	bind
50853	11	8867	7	NULL	NULL	0	NULL	statement 2	NULL		allows	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20258_s_166	7657595	A  ligand-induced three-dimensional conformation may occur upon binding of  RA to an RAR such that the ligand binding domain ```folds'''   around the ligand leaving lysine 220 and arginine 269 to interact with  the carboxylate tail and methionine 406 and, possibly, isoleucine 410,  to interact with the methyl group located at the 9 position on  9- cis-RA.	bind
50854	12	8867	7	NULL	NULL	0	NULL	statement 2	NULL		allows	NULL	possibly			statement 7	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20258_s_166	7657595	A  ligand-induced three-dimensional conformation may occur upon binding of  RA to an RAR such that the ligand binding domain ```folds'''   around the ligand leaving lysine 220 and arginine 269 to interact with  the carboxylate tail and methionine 406 and, possibly, isoleucine 410,  to interact with the methyl group located at the 9 position on  9- cis-RA.	bind
29560	1	8868	6	13	NULL	NULL	NULL	zinc finger protein	GP	maize	bind					zein gene	GP			prolamine box of promoter	NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_144_2_201_s_694	9922448	A  maize zinc-finger protein binds the prolamine box in zein gene promotors  and interacts with the basic leucine zipper transcriptional activator opaque2.	bind
29561	2	8868	6	13	NULL	NULL	NULL	statement 1	GP		interacts with					opaque 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_144_2_201_s_694	9922448	A  maize zinc-finger protein binds the prolamine box in zein gene promotors  and interacts with the basic leucine zipper transcriptional activator opaque2.	bind
29562	3	8868	6	13	NULL	NULL	NULL	opaque 2	GP		is a type of					basic leucine zipper transcriptional activator	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_144_2_201_s_694	9922448	A  maize zinc-finger protein binds the prolamine box in zein gene promotors  and interacts with the basic leucine zipper transcriptional activator opaque2.	bind
38274	1	8868	7	10	NULL	0	NULL	zinc-finger protein	NULL	maize	binds	NULL				zein gene	NULL			prolamine box of promoter	NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_144_2_201_s_694	9922448	A  maize zinc-finger protein binds the prolamine box in zein gene promotors  and interacts with the basic leucine zipper transcriptional activator opaque2.	bind
38277	2	8868	7	10	NULL	0	NULL	statement 1	NULL		interacts with	NULL				opaque2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_144_2_201_s_694	9922448	A  maize zinc-finger protein binds the prolamine box in zein gene promotors  and interacts with the basic leucine zipper transcriptional activator opaque2.	bind
38278	3	8868	7	10	NULL	0	NULL	opaque2	NULL		is a type of	NULL				basic leucine zipper transcriptional activator	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_144_2_201_s_694	9922448	A  maize zinc-finger protein binds the prolamine box in zein gene promotors  and interacts with the basic leucine zipper transcriptional activator opaque2.	bind
29563	1	8869	6	13	NULL	NULL	NULL	c-Mycax	GP		bind					promoter	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_14_8164_s_135	12808131	A  majority (603 of 1,157) of the promoters occupied by TFIID is also bound by  c-Mycax, whereas almost all the c-Myc/Max-bound promoters also harbor TFIID  in Daudi cells.	bind
29564	2	8869	6	13	NULL	NULL	NULL	c-Myc/Max	GP		bind					promoter	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_14_8164_s_135	12808131	A  majority (603 of 1,157) of the promoters occupied by TFIID is also bound by  c-Mycax, whereas almost all the c-Myc/Max-bound promoters also harbor TFIID  in Daudi cells.	bind
29565	3	8869	6	13	NULL	NULL	NULL	statement 2	Process		harbour					TFIID	GP				NULL	daudi cells	NULL	NULL	NULL	NULL	gw70_pnas_100_14_8164_s_135	12808131	A  majority (603 of 1,157) of the promoters occupied by TFIID is also bound by  c-Mycax, whereas almost all the c-Myc/Max-bound promoters also harbor TFIID  in Daudi cells.	bind
30300	4	8869	6	13	NULL	NULL	NULL	TFIID	GP		bind					promoter	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_14_8164_s_135	12808131	A  majority (603 of 1,157) of the promoters occupied by TFIID is also bound by  c-Mycax, whereas almost all the c-Myc/Max-bound promoters also harbor TFIID  in Daudi cells.	bind
30301	5	8869	6	13	NULL	NULL	NULL	statement 1	Process		occurs simultaneously with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_14_8164_s_135	12808131	A  majority (603 of 1,157) of the promoters occupied by TFIID is also bound by  c-Mycax, whereas almost all the c-Myc/Max-bound promoters also harbor TFIID  in Daudi cells.	bind
38279	1	8869	7	10	NULL	0	NULL	c-Mycax	NULL		bind	NULL					NULL			promoter	NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_14_8164_s_135	12808131	A  majority (603 of 1,157) of the promoters occupied by TFIID is also bound by  c-Mycax, whereas almost all the c-Myc/Max-bound promoters also harbor TFIID  in Daudi cells.	bind
38280	2	8869	7	10	NULL	0	NULL	 c-Myc/Max	NULL		bind	NULL					NULL			promoter	NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_14_8164_s_135	12808131	A  majority (603 of 1,157) of the promoters occupied by TFIID is also bound by  c-Mycax, whereas almost all the c-Myc/Max-bound promoters also harbor TFIID  in Daudi cells.	bind
47544	3	8869	7	10	NULL	0	NULL	TFIID	NULL		bind	NULL					NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_pnas_100_14_8164_s_135	12808131	A  majority (603 of 1,157) of the promoters occupied by TFIID is also bound by  c-Mycax, whereas almost all the c-Myc/Max-bound promoters also harbor TFIID  in Daudi cells.	bind
47545	4	8869	7	10	NULL	0	NULL	statement 1	NULL		occur simultaneously with	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_100_14_8164_s_135	12808131	A  majority (603 of 1,157) of the promoters occupied by TFIID is also bound by  c-Mycax, whereas almost all the c-Myc/Max-bound promoters also harbor TFIID  in Daudi cells.	bind
47546	5	8869	7	10	NULL	0	NULL	statement 2	NULL		harbor	NULL				TFIID	NULL				NULL	Daudi cells	0	NULL	NULL	NULL	gw70_pnas_100_14_8164_s_135	12808131	A  majority (603 of 1,157) of the promoters occupied by TFIID is also bound by  c-Mycax, whereas almost all the c-Myc/Max-bound promoters also harbor TFIID  in Daudi cells.	bind
29566	1	8870	6	13	NULL	NULL	NULL	inscuteable	GP	mammalian partner of	bind					NuMA	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_8_3144_s_380	12925752	A  mammalian partner of inscuteable binds NuMA and regulates mitotic spindle  organization.	bind
29567	2	8870	6	13	NULL	NULL	NULL	statement 1	Process		regulates					mitotic spindle	Chromosome	organization of			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_8_3144_s_380	12925752	A  mammalian partner of inscuteable binds NuMA and regulates mitotic spindle  organization.	bind
38281	1	8870	7	NULL	NULL	0	NULL	inscuteable	NULL	mammalian partner of	binds	NULL				NuMA	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_8_3144_s_380	12925752	A  mammalian partner of inscuteable binds NuMA and regulates mitotic spindle  organization.	bind
38282	2	8870	7	NULL	NULL	0	NULL	statement 1	NULL		regulates	NULL				mitotic spindle	NULL	organization of			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_8_3144_s_380	12925752	A  mammalian partner of inscuteable binds NuMA and regulates mitotic spindle  organization.	bind
29568	1	8872	6	13	NULL	NULL	NULL	cT3Ralpha	GP		bind									K14RE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_3_1416_s_93	8576132	A  mutated TREpal that does not bind cT3Ralpha  ( 28) does not  compete for the binding of cT3Ralpha  to K14RE ( Fig. 3).	bind
29569	2	8872	6	13	NULL	NULL	NULL	TREpal	GP	mutant	does not bind					cT3Ralpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_3_1416_s_93	8576132	A  mutated TREpal that does not bind cT3Ralpha  ( 28) does not  compete for the binding of cT3Ralpha  to K14RE ( Fig. 3).	bind
29570	3	8872	6	13	NULL	NULL	NULL	statement 1	Process		does not compete					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_3_1416_s_93	8576132	A  mutated TREpal that does not bind cT3Ralpha  ( 28) does not  compete for the binding of cT3Ralpha  to K14RE ( Fig. 3).	bind
38292	1	8872	7	NULL	NULL	0	NULL	TREpal	NULL	mutated	does not bind	NULL				cT3Ralpha	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_3_1416_s_93	8576132	A  mutated TREpal that does not bind cT3Ralpha  ( 28) does not  compete for the binding of cT3Ralpha  to K14RE ( Fig. 3).	bind
38293	2	8872	7	10	NULL	0	NULL	cT3Ralpha 	NULL		bind	NULL					NULL			K14RE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_3_1416_s_93	8576132	A  mutated TREpal that does not bind cT3Ralpha  ( 28) does not  compete for the binding of cT3Ralpha  to K14RE ( Fig. 3).	bind
38294	3	8872	7	10	NULL	0	NULL	statement 1			does not compete with					statement 2					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_3_1416_s_93	8576132	A  mutated TREpal that does not bind cT3Ralpha  ( 28) does not  compete for the binding of cT3Ralpha  to K14RE ( Fig. 3).	bind
29571	1	8873	6	13	NULL	NULL	NULL	PRMT5 construct	GP	mutant;; myc tagged	leads to			S-adenosyl-l-methionine-binding motif I		enzymatic activity	Process	complete loss of			NULL	COS-1 cells	NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_276_35_11413150_s_9	11413150	A  mutation introduced into the S-adenosyl-l-methionine-binding motif I of  a myc-tagged PRMT5 construct in COS-1 cells led to a near complete loss  of observed enzymatic activity.	bind
38295	1	8873	7	10	NULL	0	NULL	PRMT5 construct	NULL	myc-tagged;;mutant	leads to	NULL		S-adenosyl-l-methionine-binding motif I 		enzymatic activity	NULL	near complete loss of			NULL	COS-1 cells 	NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_276_35_11413150_s_9	11413150	A  mutation introduced into the S-adenosyl-l-methionine-binding motif I of  a myc-tagged PRMT5 construct in COS-1 cells led to a near complete loss  of observed enzymatic activity.	bind
29572	1	8879	6	13	NULL	NULL	NULL	CIS gene	GP		is induced by					cytokine	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_22_0_503_s_373	15032587	A  novel cytokine-inducible gene CIS encodes an SH2-containing protein that binds to  tyrosine-phosphorylated interleukin 3 and erythropoietin receptors.	bind
29573	2	8879	6	13	NULL	NULL	NULL	CIS gene	GP		encodes					SH2-containing protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_22_0_503_s_373	15032587	A  novel cytokine-inducible gene CIS encodes an SH2-containing protein that binds to  tyrosine-phosphorylated interleukin 3 and erythropoietin receptors.	bind
29574	3	8879	6	13	NULL	NULL	NULL	statement 2	GP		bind					interleukin 3	GP	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_22_0_503_s_373	15032587	A  novel cytokine-inducible gene CIS encodes an SH2-containing protein that binds to  tyrosine-phosphorylated interleukin 3 and erythropoietin receptors.	bind
29575	4	8879	6	13	NULL	NULL	NULL	statement 2	GP		bind					erythropoietin receptors	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_22_0_503_s_373	15032587	A  novel cytokine-inducible gene CIS encodes an SH2-containing protein that binds to  tyrosine-phosphorylated interleukin 3 and erythropoietin receptors.	bind
38297	1	8879	7	NULL	NULL	0	NULL	CIS	NULL		encode	NULL				SH2-containing protein	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_22_0_503_s_373	15032587	A  novel cytokine-inducible gene CIS encodes an SH2-containing protein that binds to  tyrosine-phosphorylated interleukin 3 and erythropoietin receptors.	bind
38298	2	8879	7	NULL	NULL	0	NULL	CIS	NULL		is	NULL				cytokine-inducible gene	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_22_0_503_s_373	15032587	A  novel cytokine-inducible gene CIS encodes an SH2-containing protein that binds to  tyrosine-phosphorylated interleukin 3 and erythropoietin receptors.	bind
38299	3	8879	7	NULL	NULL	0	NULL	SH2-containing protein	NULL		binds to	NULL				interleukin 3 	NULL	phosphorylated	tyrosine		NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_22_0_503_s_373	15032587	A  novel cytokine-inducible gene CIS encodes an SH2-containing protein that binds to  tyrosine-phosphorylated interleukin 3 and erythropoietin receptors.	bind
38300	4	8879	7	NULL	NULL	0	NULL	SH2-containing protein	NULL		binds to	NULL				erythropoietin receptor	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_22_0_503_s_373	15032587	A  novel cytokine-inducible gene CIS encodes an SH2-containing protein that binds to  tyrosine-phosphorylated interleukin 3 and erythropoietin receptors.	bind
29576	1	8880	6	13	NULL	NULL	NULL	PAR3	GP		bind		directly			PAR6	GP		PDZ domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_106_4_489_s_230	11525734	A  number of other PAR gene products have  been shown to be essential in establishing  polarity in the  C. elegans embryo, including a PDZ-containing  protein, PAR3, that binds directly to the PDZ domain  of PAR6.	bind
29577	2	8880	6	13	NULL	NULL	NULL	PAR gene products 	GP		establish					embryo	Organism	 polarity of;;C. elegans			NULL		NULL	NULL	NULL	NULL	gw60_cell_106_4_489_s_230	11525734	A  number of other PAR gene products have  been shown to be essential in establishing  polarity in the  C. elegans embryo, including a PDZ-containing  protein, PAR3, that binds directly to the PDZ domain  of PAR6.	bind
46958	3	8880	6	13	NULL	NULL	NULL	PAR3	GP		is a type of					PDZ-containing protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_106_4_489_s_230	11525734	A  number of other PAR gene products have  been shown to be essential in establishing  polarity in the  C. elegans embryo, including a PDZ-containing  protein, PAR3, that binds directly to the PDZ domain  of PAR6.	bind
38301	1	8880	7	NULL	NULL	0	NULL	 PAR3	NULL		binds	NULL	directly			PAR6	NULL		PDZ domain		NULL		0	NULL	NULL	NULL	gw60_cell_106_4_489_s_230	11525734	A  number of other PAR gene products have  been shown to be essential in establishing  polarity in the  C. elegans embryo, including a PDZ-containing  protein, PAR3, that binds directly to the PDZ domain  of PAR6.	bind
38302	2	8880	7	10	NULL	0	NULL	PAR gene products 	NULL		establishes	NULL				embryo	NULL	polarity of;;C. elegans			NULL		NULL	NULL	NULL	NULL	gw60_cell_106_4_489_s_230	11525734	A  number of other PAR gene products have  been shown to be essential in establishing  polarity in the  C. elegans embryo, including a PDZ-containing  protein, PAR3, that binds directly to the PDZ domain  of PAR6.	bind
38303	3	8880	7	NULL	NULL	0	NULL	PAR3	NULL		is a type of	NULL				PDZ-containing protein	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_106_4_489_s_230	11525734	A  number of other PAR gene products have  been shown to be essential in establishing  polarity in the  C. elegans embryo, including a PDZ-containing  protein, PAR3, that binds directly to the PDZ domain  of PAR6.	bind
29578	1	8881	6	13	NULL	NULL	NULL	virus	Organism		bind					CD4	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_41_23883_s_63	7592573	A  number of studies determined that antibodies to V3 were capable of  neutralizing virus infectivity(103-109) without affecting virus  binding to CD4( 108,  109) .	bind
29579	2	8881	6	13	NULL	NULL	NULL	antibodies to V3	GP		neutralize					virus	Organism	infectivity of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_41_23883_s_63	7592573	A  number of studies determined that antibodies to V3 were capable of  neutralizing virus infectivity(103-109) without affecting virus  binding to CD4( 108,  109) .	bind
29580	3	8881	6	13	NULL	NULL	NULL	statement 2	Process		does not affect					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_41_23883_s_63	7592573	A  number of studies determined that antibodies to V3 were capable of  neutralizing virus infectivity(103-109) without affecting virus  binding to CD4( 108,  109) .	bind
38304	1	8881	7	10	NULL	0	NULL	V3 antibodies	NULL		neutralize	NULL				virus	NULL	infectivity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_41_23883_s_63	7592573	A  number of studies determined that antibodies to V3 were capable of  neutralizing virus infectivity(103-109) without affecting virus  binding to CD4( 108,  109) .	bind
38305	2	8881	7	NULL	NULL	0	NULL	virus	NULL		bind	NULL				CD4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_41_23883_s_63	7592573	A  number of studies determined that antibodies to V3 were capable of  neutralizing virus infectivity(103-109) without affecting virus  binding to CD4( 108,  109) .	bind
38306	3	8881	7	NULL	NULL	0	NULL	statement 1	NULL		does not affect	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_41_23883_s_63	7592573	A  number of studies determined that antibodies to V3 were capable of  neutralizing virus infectivity(103-109) without affecting virus  binding to CD4( 108,  109) .	bind
29581	1	8882	6	13	NULL	NULL	NULL	pde2delta	GP	mutant	lacks					cAMP-phosphodiesterase	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7064_s_153	9819393	A  pde2delta mutant strain lacks the cAMP-phosphodiesterase responsible for conversion of the majority of cytosolic cAMP to AMP, and as a consequence, addition of exogenous cAMP to the mutant cells increases the cytosolic cAMP concentration ( 64,  71,  72).	bind
29582	2	8882	6	13	NULL	NULL	NULL	cAMP	Chemical	cytosolic	is converted to					AMP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7064_s_153	9819393	A  pde2delta mutant strain lacks the cAMP-phosphodiesterase responsible for conversion of the majority of cytosolic cAMP to AMP, and as a consequence, addition of exogenous cAMP to the mutant cells increases the cytosolic cAMP concentration ( 64,  71,  72).	bind
29583	3	8882	6	13	NULL	NULL	NULL	pde2delta	GP	mutant	is responsible for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7064_s_153	9819393	A  pde2delta mutant strain lacks the cAMP-phosphodiesterase responsible for conversion of the majority of cytosolic cAMP to AMP, and as a consequence, addition of exogenous cAMP to the mutant cells increases the cytosolic cAMP concentration ( 64,  71,  72).	bind
29584	4	8882	6	13	NULL	NULL	NULL	exogenous AMP	Chemical	addition of	increases					cAMP	Chemical	concentration of;; cytosolic			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7064_s_153	9819393	A  pde2delta mutant strain lacks the cAMP-phosphodiesterase responsible for conversion of the majority of cytosolic cAMP to AMP, and as a consequence, addition of exogenous cAMP to the mutant cells increases the cytosolic cAMP concentration ( 64,  71,  72).	bind
38307	1	8882	7	NULL	NULL	0	NULL	pde2delta	NULL	mutant	lacks	NULL				cAMP-phosphodiesterase	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_12_7064_s_153	9819393	A  pde2delta mutant strain lacks the cAMP-phosphodiesterase responsible for conversion of the majority of cytosolic cAMP to AMP, and as a consequence, addition of exogenous cAMP to the mutant cells increases the cytosolic cAMP concentration ( 64,  71,  72).	bind
38308	2	8882	7	NULL	NULL	0	NULL	cAMP	NULL	cytosolic	converts to	NULL				AMP	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_12_7064_s_153	9819393	A  pde2delta mutant strain lacks the cAMP-phosphodiesterase responsible for conversion of the majority of cytosolic cAMP to AMP, and as a consequence, addition of exogenous cAMP to the mutant cells increases the cytosolic cAMP concentration ( 64,  71,  72).	bind
38309	3	8882	7	NULL	NULL	0	NULL	statement 1	NULL		responsible for	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_12_7064_s_153	9819393	A  pde2delta mutant strain lacks the cAMP-phosphodiesterase responsible for conversion of the majority of cytosolic cAMP to AMP, and as a consequence, addition of exogenous cAMP to the mutant cells increases the cytosolic cAMP concentration ( 64,  71,  72).	bind
38310	4	8882	7	10	NULL	0	NULL	exogenous cAMP	NULL	addition of	increase	NULL				cAMP	NULL	concentration of;;cytosolic			NULL	mutant cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7064_s_153	9819393	A  pde2delta mutant strain lacks the cAMP-phosphodiesterase responsible for conversion of the majority of cytosolic cAMP to AMP, and as a consequence, addition of exogenous cAMP to the mutant cells increases the cytosolic cAMP concentration ( 64,  71,  72).	bind
38311	5	8882	7	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_12_7064_s_153	9819393	A  pde2delta mutant strain lacks the cAMP-phosphodiesterase responsible for conversion of the majority of cytosolic cAMP to AMP, and as a consequence, addition of exogenous cAMP to the mutant cells increases the cytosolic cAMP concentration ( 64,  71,  72).	bind
29585	1	8883	6	13	NULL	NULL	NULL	peptide	GP		bind			Rev activation domain		CRM1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_2_255_s_200	10209022	A  peptide comprising the Rev activation domain plus a few  flanking residues bound CRM1 700 times weakerR ( Kd   7 muM), and the minimum Rev activation domain itself even  5,000-fold weaker ( Kd   50 muM) than snurportin 1.	bind
29586	2	8883	6	13	NULL	NULL	NULL	snurportin 1	GP		bind					CRM1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_2_255_s_200	10209022	A  peptide comprising the Rev activation domain plus a few  flanking residues bound CRM1 700 times weakerR ( Kd   7 muM), and the minimum Rev activation domain itself even  5,000-fold weaker ( Kd   50 muM) than snurportin 1.	bind
29587	3	8883	6	13	NULL	NULL	NULL	statement 1	Process	affinity of	is less than					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_2_255_s_200	10209022	A  peptide comprising the Rev activation domain plus a few  flanking residues bound CRM1 700 times weakerR ( Kd   7 muM), and the minimum Rev activation domain itself even  5,000-fold weaker ( Kd   50 muM) than snurportin 1.	bind
38312	1	8883	7	NULL	NULL	0	NULL	peptide	NULL		bind	NULL		Rev activation domain plus a few flanking residues		CRM1	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_2_255_s_200	10209022	A  peptide comprising the Rev activation domain plus a few  flanking residues bound CRM1 700 times weakerR ( Kd   7 muM), and the minimum Rev activation domain itself even  5,000-fold weaker ( Kd   50 muM) than snurportin 1.	bind
38313	2	8883	7	NULL	NULL	0	NULL	peptide	NULL		bind	NULL		Rev activation domain		CRM1	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_2_255_s_200	10209022	A  peptide comprising the Rev activation domain plus a few  flanking residues bound CRM1 700 times weakerR ( Kd   7 muM), and the minimum Rev activation domain itself even  5,000-fold weaker ( Kd   50 muM) than snurportin 1.	bind
38314	3	8883	7	NULL	NULL	0	NULL	snurportin 1	NULL		bind	NULL				CRM1	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_2_255_s_200	10209022	A  peptide comprising the Rev activation domain plus a few  flanking residues bound CRM1 700 times weakerR ( Kd   7 muM), and the minimum Rev activation domain itself even  5,000-fold weaker ( Kd   50 muM) than snurportin 1.	bind
38315	4	8883	7	NULL	NULL	0	NULL	statement 1	NULL	binding of	is weaker than	NULL				statement 3	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_2_255_s_200	10209022	A  peptide comprising the Rev activation domain plus a few  flanking residues bound CRM1 700 times weakerR ( Kd   7 muM), and the minimum Rev activation domain itself even  5,000-fold weaker ( Kd   50 muM) than snurportin 1.	bind
38316	5	8883	7	NULL	NULL	0	NULL	statement 2	NULL	binding of	is weaker than	NULL				statement 3	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_2_255_s_200	10209022	A  peptide comprising the Rev activation domain plus a few  flanking residues bound CRM1 700 times weakerR ( Kd   7 muM), and the minimum Rev activation domain itself even  5,000-fold weaker ( Kd   50 muM) than snurportin 1.	bind
29588	1	8884	6	13	NULL	NULL	NULL	PhoP	GP		bind					PV	GP			core binding region of promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_187_15_5166_s_195	16030210	A  phoB promoter fragment containing only the PS promoter (from pPS2 [Fig.  1]) was used as a template for in vitro transcription to determine if reduction of the PS transcript from the  phoB-PS+V promoter in the presence of phosphorylated PhoP was exclusively the result of PhoP binding to the PV promoter core binding region, which blocked RNAP passage (Fig.  5A, top panel).	bind
29589	2	8884	6	13	NULL	NULL	NULL	statement 1	Process		blocks					RNAP	GP	passage of 			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_187_15_5166_s_195	16030210	A  phoB promoter fragment containing only the PS promoter (from pPS2 [Fig.  1]) was used as a template for in vitro transcription to determine if reduction of the PS transcript from the  phoB-PS+V promoter in the presence of phosphorylated PhoP was exclusively the result of PhoP binding to the PV promoter core binding region, which blocked RNAP passage (Fig.  5A, top panel).	bind
38317	1	8884	7	NULL	NULL	0	NULL	PhoP	NULL		bind	NULL				PV	NULL			promoter core binding region	NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_15_5166_s_195	16030210	A  phoB promoter fragment containing only the PS promoter (from pPS2 [Fig.  1]) was used as a template for in vitro transcription to determine if reduction of the PS transcript from the  phoB-PS+V promoter in the presence of phosphorylated PhoP was exclusively the result of PhoP binding to the PV promoter core binding region, which blocked RNAP passage (Fig.  5A, top panel).	bind
38318	2	8884	7	10	NULL	0	NULL	statement 1	NULL		blocks	NULL				RNAP	NULL	passage of			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_187_15_5166_s_195	16030210	A  phoB promoter fragment containing only the PS promoter (from pPS2 [Fig.  1]) was used as a template for in vitro transcription to determine if reduction of the PS transcript from the  phoB-PS+V promoter in the presence of phosphorylated PhoP was exclusively the result of PhoP binding to the PV promoter core binding region, which blocked RNAP passage (Fig.  5A, top panel).	bind
29612	1	8885	6	13	NULL	NULL	NULL	Cbl	GP		bind					Crk	GP		SH2 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_14_8435_s_7	8626543	A  phosphopeptide corresponding to a potential Crk SH2 domain-binding  motif in Cbl (pYDVP) specifically inhibited binding between Cbl and Crk  SH2 domain.	bind
29693	2	8885	6	13	NULL	NULL	NULL	phosphopeptide	GP		corresponds to					Cbl	GP	potential	Crk SH2 domain-binding motif		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_14_8435_s_7	8626543	A  phosphopeptide corresponding to a potential Crk SH2 domain-binding  motif in Cbl (pYDVP) specifically inhibited binding between Cbl and Crk  SH2 domain.	bind
29695	3	8885	6	13	NULL	NULL	NULL	statement 2	Process		inhibits					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_14_8435_s_7	8626543	A  phosphopeptide corresponding to a potential Crk SH2 domain-binding  motif in Cbl (pYDVP) specifically inhibited binding between Cbl and Crk  SH2 domain.	bind
38319	1	8885	7	NULL	NULL	0	NULL	Cbl	NULL		bind	NULL				Crk	NULL		SH2 domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8435_s_7	8626543	A  phosphopeptide corresponding to a potential Crk SH2 domain-binding  motif in Cbl (pYDVP) specifically inhibited binding between Cbl and Crk  SH2 domain.	bind
38320	2	8885	7	NULL	NULL	0	NULL	phosphopeptide	NULL		corresponds to	NULL				Cbl	NULL		pYDVP Crk SH2 domain-binding motif		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_14_8435_s_7	8626543	A  phosphopeptide corresponding to a potential Crk SH2 domain-binding  motif in Cbl (pYDVP) specifically inhibited binding between Cbl and Crk  SH2 domain.	bind
38321	3	8885	7	NULL	NULL	0	NULL	statement 2	NULL		inhibits	NULL	specifically			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8435_s_7	8626543	A  phosphopeptide corresponding to a potential Crk SH2 domain-binding  motif in Cbl (pYDVP) specifically inhibited binding between Cbl and Crk  SH2 domain.	bind
29696	1	8886	6	13	NULL	NULL	NULL	v-Crk	GP		bind					paxillin	GP	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31219_s_7	8537387	A  phosphotyrosine peptide, which can inhibit v-Crk binding to paxillin,  did not inhibit Csk binding to paxillin, suggesting that v-Crk and Csk  bind to different tyrosine-phosphorylated sites in paxillin.	bind
29697	2	8886	6	13	NULL	NULL	NULL	Csk	GP		bind					paxillin	GP	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31219_s_7	8537387	A  phosphotyrosine peptide, which can inhibit v-Crk binding to paxillin,  did not inhibit Csk binding to paxillin, suggesting that v-Crk and Csk  bind to different tyrosine-phosphorylated sites in paxillin.	bind
29698	3	8886	6	13	NULL	NULL	NULL	phosphotyrosine peptide	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31219_s_7	8537387	A  phosphotyrosine peptide, which can inhibit v-Crk binding to paxillin,  did not inhibit Csk binding to paxillin, suggesting that v-Crk and Csk  bind to different tyrosine-phosphorylated sites in paxillin.	bind
29699	4	8886	6	13	NULL	NULL	NULL	phosphotyrosine peptide	GP		does not inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31219_s_7	8537387	A  phosphotyrosine peptide, which can inhibit v-Crk binding to paxillin,  did not inhibit Csk binding to paxillin, suggesting that v-Crk and Csk  bind to different tyrosine-phosphorylated sites in paxillin.	bind
38402	1	8886	7	10	NULL	0	NULL	v-Crk	NULL		bind	NULL				paxillin	NULL	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31219_s_7	8537387	A  phosphotyrosine peptide, which can inhibit v-Crk binding to paxillin,  did not inhibit Csk binding to paxillin, suggesting that v-Crk and Csk  bind to different tyrosine-phosphorylated sites in paxillin.	bind
38403	2	8886	7	10	NULL	0	NULL	Csk	NULL		bind	NULL				paxillin	NULL	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31219_s_7	8537387	A  phosphotyrosine peptide, which can inhibit v-Crk binding to paxillin,  did not inhibit Csk binding to paxillin, suggesting that v-Crk and Csk  bind to different tyrosine-phosphorylated sites in paxillin.	bind
38404	3	8886	7	NULL	NULL	0	NULL	phosphotyrosine peptide	NULL		inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31219_s_7	8537387	A  phosphotyrosine peptide, which can inhibit v-Crk binding to paxillin,  did not inhibit Csk binding to paxillin, suggesting that v-Crk and Csk  bind to different tyrosine-phosphorylated sites in paxillin.	bind
38405	4	8886	7	NULL	NULL	0	NULL	phosphotyrosine peptide	NULL		does not inhibit	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31219_s_7	8537387	A  phosphotyrosine peptide, which can inhibit v-Crk binding to paxillin,  did not inhibit Csk binding to paxillin, suggesting that v-Crk and Csk  bind to different tyrosine-phosphorylated sites in paxillin.	bind
38406	5	8886	7	NULL	NULL	0	NULL	statement 1	NULL	binding site of	is different from	NULL				statement 2	NULL	binding site of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31219_s_7	8537387	A  phosphotyrosine peptide, which can inhibit v-Crk binding to paxillin,  did not inhibit Csk binding to paxillin, suggesting that v-Crk and Csk  bind to different tyrosine-phosphorylated sites in paxillin.	bind
29700	1	8887	6	13	NULL	NULL	NULL	Pex6p	GP		bind					Pex15p	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_6_2226_s_7	12808025	A  point mutation in the Walker A motif of D1 (K489A) decreased the binding of  Pex6p to Pex15p indicating that the interaction of Pex6p with Pex15p required  binding of ATP.	bind
29701	2	8887	6	13	NULL	NULL	NULL	D1	GP	point mutant	decreases			Walker A motif (K489A)		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_6_2226_s_7	12808025	A  point mutation in the Walker A motif of D1 (K489A) decreased the binding of  Pex6p to Pex15p indicating that the interaction of Pex6p with Pex15p required  binding of ATP.	bind
29702	3	8887	6	13	NULL	NULL	NULL	statement 1	Process		requires					ATP	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_6_2226_s_7	12808025	A  point mutation in the Walker A motif of D1 (K489A) decreased the binding of  Pex6p to Pex15p indicating that the interaction of Pex6p with Pex15p required  binding of ATP.	bind
38407	1	8887	7	NULL	NULL	0	NULL	Pex6p	NULL		bind	NULL				 Pex15p	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_6_2226_s_7	12808025	A  point mutation in the Walker A motif of D1 (K489A) decreased the binding of  Pex6p to Pex15p indicating that the interaction of Pex6p with Pex15p required  binding of ATP.	bind
38408	2	8887	7	NULL	NULL	0	NULL	D1	NULL	point mutant	decrease	NULL		Walker A motif K489A		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_6_2226_s_7	12808025	A  point mutation in the Walker A motif of D1 (K489A) decreased the binding of  Pex6p to Pex15p indicating that the interaction of Pex6p with Pex15p required  binding of ATP.	bind
38409	3	8887	7	NULL	NULL	0	NULL	statement 1	NULL		requires	NULL				ATP	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_6_2226_s_7	12808025	A  point mutation in the Walker A motif of D1 (K489A) decreased the binding of  Pex6p to Pex15p indicating that the interaction of Pex6p with Pex15p required  binding of ATP.	bind
29703	1	8888	6	13	NULL	NULL	NULL	Oct-1	GP		bind					TNF	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_annurevgenomicshum_2_0_373_s_643	null	A  polymorphism that affects OCT-1 binding to the TNF promoter region is associated  with severe malaria.	bind
29837	2	8888	6	13	NULL	NULL	NULL	gene polymorphism	Process		is associated with					severe malaria	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw70_annurevgenomicshum_2_0_373_s_643	null	A  polymorphism that affects OCT-1 binding to the TNF promoter region is associated  with severe malaria.	bind
29838	3	8888	6	13	NULL	NULL	NULL	statement 2	Process		affects					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevgenomicshum_2_0_373_s_643	null	A  polymorphism that affects OCT-1 binding to the TNF promoter region is associated  with severe malaria.	bind
38410	1	8888	7	NULL	NULL	0	NULL	OCT-1	NULL		bind	NULL				TNF	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_annurevgenomicshum_2_0_373_s_643	null	A  polymorphism that affects OCT-1 binding to the TNF promoter region is associated  with severe malaria.	bind
38411	2	8888	7	NULL	NULL	0	NULL	polymorphism	NULL		affects	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevgenomicshum_2_0_373_s_643	null	A  polymorphism that affects OCT-1 binding to the TNF promoter region is associated  with severe malaria.	bind
38412	3	8888	7	NULL	NULL	0	NULL	statement 2	NULL		is associated with	NULL				malaria	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevgenomicshum_2_0_373_s_643	null	A  polymorphism that affects OCT-1 binding to the TNF promoter region is associated  with severe malaria.	bind
29704	1	8889	6	13	NULL	NULL	NULL	FK506	Chemical		bind					FKBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_89_6_875_s_118	9200606	A  portion of FK506 bound to FKBP, and the AlaPro dipeptides bound to Pin1  and CyPA are shown.	bind
29705	2	8889	6	13	NULL	NULL	NULL	AlaPro dipeptide	AminoAcid		bind					Pin1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_89_6_875_s_118	9200606	A  portion of FK506 bound to FKBP, and the AlaPro dipeptides bound to Pin1  and CyPA are shown.	bind
29708	3	8889	6	13	NULL	NULL	NULL	AlaPro dipeptide	AminoAcid		bind					CyPA	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_89_6_875_s_118	9200606	A  portion of FK506 bound to FKBP, and the AlaPro dipeptides bound to Pin1  and CyPA are shown.	bind
38413	1	8889	7	10	NULL	0	NULL	FK506	NULL		bind	NULL				FKBP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cell_89_6_875_s_118	9200606	A  portion of FK506 bound to FKBP, and the AlaPro dipeptides bound to Pin1  and CyPA are shown.	bind
38414	2	8889	7	NULL	NULL	0	NULL	AlaPro dipeptides	NULL		bind	NULL				Pin1	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_89_6_875_s_118	9200606	A  portion of FK506 bound to FKBP, and the AlaPro dipeptides bound to Pin1  and CyPA are shown.	bind
38415	3	8889	7	NULL	NULL	0	NULL	AlaPro dipeptides	NULL		bind	NULL				CyPA	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_89_6_875_s_118	9200606	A  portion of FK506 bound to FKBP, and the AlaPro dipeptides bound to Pin1  and CyPA are shown.	bind
29709	1	8890	6	13	NULL	NULL	NULL	fMLP	GP		bind					fMLP receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_305_3_846_s_130	12626661	A  previous study (Raiden et al.,  1997  ) reported that losartan blocked the binding of  [3]fMLP to the fMLP receptor, which was found to have 25 to 30%  structural homology with the AT1 receptor.	bind
29711	2	8890	6	13	NULL	NULL	NULL	losartan	Chemical		blocked					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_305_3_846_s_130	12626661	A  previous study (Raiden et al.,  1997  ) reported that losartan blocked the binding of  [3]fMLP to the fMLP receptor, which was found to have 25 to 30%  structural homology with the AT1 receptor.	bind
29714	3	8890	6	13	NULL	NULL	NULL	fMLP receptor	GP		is homologous to		structurally			AT1 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_305_3_846_s_130	12626661	A  previous study (Raiden et al.,  1997  ) reported that losartan blocked the binding of  [3]fMLP to the fMLP receptor, which was found to have 25 to 30%  structural homology with the AT1 receptor.	bind
38416	1	8890	7	10	NULL	0	NULL	fMLP 			bind					fMLP receptor					NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_305_3_846_s_130	12626661	A  previous study (Raiden et al.,  1997  ) reported that losartan blocked the binding of  [3]fMLP to the fMLP receptor, which was found to have 25 to 30%  structural homology with the AT1 receptor.	bind
38417	2	8890	7	NULL	NULL	0	NULL	losartan 	NULL		block	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_305_3_846_s_130	12626661	A  previous study (Raiden et al.,  1997  ) reported that losartan blocked the binding of  [3]fMLP to the fMLP receptor, which was found to have 25 to 30%  structural homology with the AT1 receptor.	bind
38418	3	8890	7	10	NULL	0	NULL	losartan 			is homologous to		structurally			AT1 receptor					NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_305_3_846_s_130	12626661	A  previous study (Raiden et al.,  1997  ) reported that losartan blocked the binding of  [3]fMLP to the fMLP receptor, which was found to have 25 to 30%  structural homology with the AT1 receptor.	bind
29717	1	8891	6	13	NULL	NULL	NULL	calponin	GP		bind			CH domain		actin	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-mol-biol_359_2_16626733_s_5	16626733	A  previous three-dimensional reconstruction of the calponin-F-actin complex  has led to the conclusion that the visualized portion of calponin bound  to actin belongs to its amino-terminal homology (CH) domain.	bind
29718	2	8891	6	13	NULL	NULL	NULL	CH domain	GP		is					amino-terminal homology domain	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-mol-biol_359_2_16626733_s_5	16626733	A  previous three-dimensional reconstruction of the calponin-F-actin complex  has led to the conclusion that the visualized portion of calponin bound  to actin belongs to its amino-terminal homology (CH) domain.	bind
38419	1	8891	7	10	NULL	0	NULL	calponin			bind			CH domain		actin					NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-mol-biol_359_2_16626733_s_5	16626733	A  previous three-dimensional reconstruction of the calponin-F-actin complex  has led to the conclusion that the visualized portion of calponin bound  to actin belongs to its amino-terminal homology (CH) domain.	bind
56166	2	8891	7	10	NULL	0	NULL	CH domain			is					amino-terminal homology domain					NULL		0	NULL	NULL	NULL	abs-batch0680-0699_j-mol-biol_359_2_16626733_s_5	16626733	A  previous three-dimensional reconstruction of the calponin-F-actin complex  has led to the conclusion that the visualized portion of calponin bound  to actin belongs to its amino-terminal homology (CH) domain.	bind
29719	1	8892	6	13	NULL	NULL	NULL	VWF	GP	proteolytic fragment of	bind		directly	Leu-480/Val-481 to Gly-718		GPIb	GP	platelet			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_22_13406_s_25	7539426	A  proteolytic fragment of VWF that contains residues Leu-480/Val-481 to  Gly-718  ( 7) binds directly to platelet GPIb.	bind
38420	1	8892	7	10	NULL	0	NULL	VWF	NULL	proteolytic fragment of	bind	NULL	directly	Leu-480/Val-481 to Gly-718		GPIb	NULL	platelet			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_22_13406_s_25	7539426	A  proteolytic fragment of VWF that contains residues Leu-480/Val-481 to  Gly-718  ( 7) binds directly to platelet GPIb.	bind
29839	1	8893	6	13	NULL	NULL	NULL	fusion protein	GP	purified	bind			 A subunit residues 328-390		CaN	GP		B subunit		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_456_s_5	7814411	A  purified fusion protein containing residues 328-390 of the A  subunit 1) binds CaN B subunit, and 2) inhibits (IC   =  0.1 muM) the  in vitro  stimulation  of CaN A phosphatase activity by purified CaN B subunit.	bind
29841	2	8893	6	13	NULL	NULL	NULL	CaN	GP	purified	stimulates			B subunit		CaN A	GP	phosphatase activity of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_456_s_5	7814411	A  purified fusion protein containing residues 328-390 of the A  subunit 1) binds CaN B subunit, and 2) inhibits (IC   =  0.1 muM) the  in vitro  stimulation  of CaN A phosphatase activity by purified CaN B subunit.	bind
29842	3	8893	6	13	NULL	NULL	NULL	statement 1	Process		inhibits					statement 3	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_456_s_5	7814411	A  purified fusion protein containing residues 328-390 of the A  subunit 1) binds CaN B subunit, and 2) inhibits (IC   =  0.1 muM) the  in vitro  stimulation  of CaN A phosphatase activity by purified CaN B subunit.	bind
38422	1	8893	7	10	NULL	0	NULL	fusion protein		purified	binds			A subunit residues 328-390		CaN			B subunit		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_456_s_5	7814411	A  purified fusion protein containing residues 328-390 of the A  subunit 1) binds CaN B subunit, and 2) inhibits (IC   =  0.1 muM) the  in vitro  stimulation  of CaN A phosphatase activity by purified CaN B subunit.	bind
38423	2	8893	7	10	NULL	0	NULL	CaN	NULL	purified	stimulates	NULL		B subunit		CaN A 	NULL	phosphatase activity of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_456_s_5	7814411	A  purified fusion protein containing residues 328-390 of the A  subunit 1) binds CaN B subunit, and 2) inhibits (IC   =  0.1 muM) the  in vitro  stimulation  of CaN A phosphatase activity by purified CaN B subunit.	bind
38424	3	8893	7	10	NULL	0	NULL	statement 1			inhibits					statement 2					NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_456_s_5	7814411	A  purified fusion protein containing residues 328-390 of the A  subunit 1) binds CaN B subunit, and 2) inhibits (IC   =  0.1 muM) the  in vitro  stimulation  of CaN A phosphatase activity by purified CaN B subunit.	bind
29720	1	8894	6	13	NULL	NULL	NULL	SOM230	Chemical		is a type of					cyclohexapeptide somatostatin analog	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-endocrinol-invest_28_11-suppl_16625840_s_3	16625840	A  rational medicinal chemistry approach capitalising on structure activity  relationships has led to the discovery of SOM230, a novel, stable cyclohexapeptide  somatostatin analog which exhibits multi-receptor binding to human somatostatin  receptor (SSTR) subtypes (SSTR 1-5).	bind
29721	2	8894	6	13	NULL	NULL	NULL	SSTR 1-5	GP		is a type of					somatostatin receptor subtype	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-endocrinol-invest_28_11-suppl_16625840_s_3	16625840	A  rational medicinal chemistry approach capitalising on structure activity  relationships has led to the discovery of SOM230, a novel, stable cyclohexapeptide  somatostatin analog which exhibits multi-receptor binding to human somatostatin  receptor (SSTR) subtypes (SSTR 1-5).	bind
29722	3	8894	6	13	NULL	NULL	NULL	SOM230	Chemical		bind					SSTR 1-5	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-endocrinol-invest_28_11-suppl_16625840_s_3	16625840	A  rational medicinal chemistry approach capitalising on structure activity  relationships has led to the discovery of SOM230, a novel, stable cyclohexapeptide  somatostatin analog which exhibits multi-receptor binding to human somatostatin  receptor (SSTR) subtypes (SSTR 1-5).	bind
38425	1	8894	7	NULL	NULL	0	NULL	SOM230	NULL		exhibits	NULL				 multi-receptor binding	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-endocrinol-invest_28_11-suppl_16625840_s_3	16625840	A  rational medicinal chemistry approach capitalising on structure activity  relationships has led to the discovery of SOM230, a novel, stable cyclohexapeptide  somatostatin analog which exhibits multi-receptor binding to human somatostatin  receptor (SSTR) subtypes (SSTR 1-5).	bind
38426	2	8894	7	NULL	NULL	0	NULL	SOM230	NULL		bind	NULL				SSTR1	NULL	human			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-endocrinol-invest_28_11-suppl_16625840_s_3	16625840	A  rational medicinal chemistry approach capitalising on structure activity  relationships has led to the discovery of SOM230, a novel, stable cyclohexapeptide  somatostatin analog which exhibits multi-receptor binding to human somatostatin  receptor (SSTR) subtypes (SSTR 1-5).	bind
38427	3	8894	7	NULL	NULL	0	NULL	SOM230	NULL		bind	NULL				SSTR2	NULL	human			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-endocrinol-invest_28_11-suppl_16625840_s_3	16625840	A  rational medicinal chemistry approach capitalising on structure activity  relationships has led to the discovery of SOM230, a novel, stable cyclohexapeptide  somatostatin analog which exhibits multi-receptor binding to human somatostatin  receptor (SSTR) subtypes (SSTR 1-5).	bind
38428	4	8894	7	NULL	NULL	0	NULL	SOM230	NULL		bind	NULL				SSTR3	NULL	human			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-endocrinol-invest_28_11-suppl_16625840_s_3	16625840	A  rational medicinal chemistry approach capitalising on structure activity  relationships has led to the discovery of SOM230, a novel, stable cyclohexapeptide  somatostatin analog which exhibits multi-receptor binding to human somatostatin  receptor (SSTR) subtypes (SSTR 1-5).	bind
38429	5	8894	7	NULL	NULL	0	NULL	SOM230	NULL		bind	NULL				SSTR4	NULL	human			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-endocrinol-invest_28_11-suppl_16625840_s_3	16625840	A  rational medicinal chemistry approach capitalising on structure activity  relationships has led to the discovery of SOM230, a novel, stable cyclohexapeptide  somatostatin analog which exhibits multi-receptor binding to human somatostatin  receptor (SSTR) subtypes (SSTR 1-5).	bind
38430	6	8894	7	NULL	NULL	0	NULL	SOM230	NULL		bind	NULL				SSTR5	NULL	human			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-endocrinol-invest_28_11-suppl_16625840_s_3	16625840	A  rational medicinal chemistry approach capitalising on structure activity  relationships has led to the discovery of SOM230, a novel, stable cyclohexapeptide  somatostatin analog which exhibits multi-receptor binding to human somatostatin  receptor (SSTR) subtypes (SSTR 1-5).	bind
38431	7	8894	7	NULL	NULL	0	NULL	SSTR	NULL		is	NULL				somatostatin receptor	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-endocrinol-invest_28_11-suppl_16625840_s_3	16625840	A  rational medicinal chemistry approach capitalising on structure activity  relationships has led to the discovery of SOM230, a novel, stable cyclohexapeptide  somatostatin analog which exhibits multi-receptor binding to human somatostatin  receptor (SSTR) subtypes (SSTR 1-5).	bind
38432	8	8894	7	10	NULL	0	NULL	SOM230			is an analog of		stable			cyclohexapeptide somatostatin					NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-endocrinol-invest_28_11-suppl_16625840_s_3	16625840	A  rational medicinal chemistry approach capitalising on structure activity  relationships has led to the discovery of SOM230, a novel, stable cyclohexapeptide  somatostatin analog which exhibits multi-receptor binding to human somatostatin  receptor (SSTR) subtypes (SSTR 1-5).	bind
47902	9	8894	7	NULL	NULL	0	NULL	SSTR1	NULL		is a type of	NULL				somatostatin receptor subtype	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-endocrinol-invest_28_11-suppl_16625840_s_3	16625840	A  rational medicinal chemistry approach capitalising on structure activity  relationships has led to the discovery of SOM230, a novel, stable cyclohexapeptide  somatostatin analog which exhibits multi-receptor binding to human somatostatin  receptor (SSTR) subtypes (SSTR 1-5).	bind
47903	10	8894	7	NULL	NULL	0	NULL	SSTR2	NULL		is a type of	NULL				somatostatin receptor subtype	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-endocrinol-invest_28_11-suppl_16625840_s_3	16625840	A  rational medicinal chemistry approach capitalising on structure activity  relationships has led to the discovery of SOM230, a novel, stable cyclohexapeptide  somatostatin analog which exhibits multi-receptor binding to human somatostatin  receptor (SSTR) subtypes (SSTR 1-5).	bind
47904	11	8894	7	NULL	NULL	0	NULL	SSTR3	NULL		is a type of	NULL				somatostatin receptor subtype	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-endocrinol-invest_28_11-suppl_16625840_s_3	16625840	A  rational medicinal chemistry approach capitalising on structure activity  relationships has led to the discovery of SOM230, a novel, stable cyclohexapeptide  somatostatin analog which exhibits multi-receptor binding to human somatostatin  receptor (SSTR) subtypes (SSTR 1-5).	bind
47905	12	8894	7	NULL	NULL	0	NULL	SSTR4	NULL		is a type of	NULL				somatostatin receptor subtype	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-endocrinol-invest_28_11-suppl_16625840_s_3	16625840	A  rational medicinal chemistry approach capitalising on structure activity  relationships has led to the discovery of SOM230, a novel, stable cyclohexapeptide  somatostatin analog which exhibits multi-receptor binding to human somatostatin  receptor (SSTR) subtypes (SSTR 1-5).	bind
47906	13	8894	7	NULL	NULL	0	NULL	SSTR5	NULL		is a type of	NULL				somatostatin receptor subtype	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-endocrinol-invest_28_11-suppl_16625840_s_3	16625840	A  rational medicinal chemistry approach capitalising on structure activity  relationships has led to the discovery of SOM230, a novel, stable cyclohexapeptide  somatostatin analog which exhibits multi-receptor binding to human somatostatin  receptor (SSTR) subtypes (SSTR 1-5).	bind
29843	1	8895	6	13	NULL	NULL	NULL	Raf	GP	mutant	lacks								cysteine-rich domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_17_9809_s_77	7730360	A  recent investigation has demonstrated partially reduced coprecipitation  and   in vitro binding between Ras and a Raf mutant lacking the  cysteine-rich domain  ( 28) , supporting our finding of two Ras  binding sites in Raf.	bind
30302	2	8895	6	13	NULL	NULL	NULL	Ras	GP		bind					statement 1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_17_9809_s_77	7730360	A  recent investigation has demonstrated partially reduced coprecipitation  and   in vitro binding between Ras and a Raf mutant lacking the  cysteine-rich domain  ( 28) , supporting our finding of two Ras  binding sites in Raf.	bind
30304	3	8895	6	13	NULL	NULL	NULL	Raf	GP		possesses								Ras binding site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_17_9809_s_77	7730360	A  recent investigation has demonstrated partially reduced coprecipitation  and   in vitro binding between Ras and a Raf mutant lacking the  cysteine-rich domain  ( 28) , supporting our finding of two Ras  binding sites in Raf.	bind
38433	2	8895	7	10	NULL	0	NULL	Ras	NULL		bind	NULL				statement 1	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_17_9809_s_77	7730360	A  recent investigation has demonstrated partially reduced coprecipitation  and   in vitro binding between Ras and a Raf mutant lacking the  cysteine-rich domain  ( 28) , supporting our finding of two Ras  binding sites in Raf.	bind
38434	3	8895	7	10	NULL	0	NULL	Raf	NULL		contains	NULL					NULL		Ras binding site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_17_9809_s_77	7730360	A  recent investigation has demonstrated partially reduced coprecipitation  and   in vitro binding between Ras and a Raf mutant lacking the  cysteine-rich domain  ( 28) , supporting our finding of two Ras  binding sites in Raf.	bind
46999	1	8895	7	10	NULL	0	NULL	Raf	NULL	mutant	lacks	NULL					NULL		cysteine-rich domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_17_9809_s_77	7730360	A  recent investigation has demonstrated partially reduced coprecipitation  and   in vitro binding between Ras and a Raf mutant lacking the  cysteine-rich domain  ( 28) , supporting our finding of two Ras  binding sites in Raf.	bind
29723	1	8896	6	13	NULL	NULL	NULL	Nedd4-2	GP		bind		strongly	WW3		ENaC	GP		PY motif		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_22_20019_s_294	12654927	A  recent report, published after submission of our manuscript  ( ), supports the trend we  find here, in that WW3* of Nedd4-2 binds most strongly to the ENaC PY motifs,  followed by WW4.	bind
29724	2	8896	6	13	NULL	NULL	NULL	Nedd4-2	GP		bind			WW4		ENaC	GP		PY motif		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_22_20019_s_294	12654927	A  recent report, published after submission of our manuscript  ( ), supports the trend we  find here, in that WW3* of Nedd4-2 binds most strongly to the ENaC PY motifs,  followed by WW4.	bind
38435	1	8896	7	NULL	NULL	0	NULL	 Nedd4-2	NULL		binds	NULL	strongly	WW3		 ENaC	NULL		PY motifs		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_22_20019_s_294	12654927	A  recent report, published after submission of our manuscript  ( ), supports the trend we  find here, in that WW3* of Nedd4-2 binds most strongly to the ENaC PY motifs,  followed by WW4.	bind
38436	2	8896	7	NULL	NULL	0	NULL	Nedd4-2	NULL		bind	NULL		WW4		ENaC	NULL		PY motifs		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_22_20019_s_294	12654927	A  recent report, published after submission of our manuscript  ( ), supports the trend we  find here, in that WW3* of Nedd4-2 binds most strongly to the ENaC PY motifs,  followed by WW4.	bind
29725	1	8898	6	13	NULL	NULL	NULL	rgpA kgp hagA	GP	triple mutant	does not exhibit					hemagglutination	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17955_s_11	10364243	A  rgpA kgp hagA triple mutant constructed in this study exhibited no hemagglutination using sheep erythrocytes or hemoglobin binding activity, as determined by a solid-phase binding assay with horseradish peroxidase-conjugated human hemoglobin, indicating that the adhesin domains seem to be particularly important for  P. gingivalis cells to agglutinate erythrocytes and bind hemoglobin, leading to heme acquisition.	bind
29726	2	8898	6	13	NULL	NULL	NULL	P. gingivalis cells	Cell		agglutinate					erythrocytes	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17955_s_11	10364243	A  rgpA kgp hagA triple mutant constructed in this study exhibited no hemagglutination using sheep erythrocytes or hemoglobin binding activity, as determined by a solid-phase binding assay with horseradish peroxidase-conjugated human hemoglobin, indicating that the adhesin domains seem to be particularly important for  P. gingivalis cells to agglutinate erythrocytes and bind hemoglobin, leading to heme acquisition.	bind
29727	3	8898	6	13	NULL	NULL	NULL	P. gingivalis cells	Cell		bind					hemoglobin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17955_s_11	10364243	A  rgpA kgp hagA triple mutant constructed in this study exhibited no hemagglutination using sheep erythrocytes or hemoglobin binding activity, as determined by a solid-phase binding assay with horseradish peroxidase-conjugated human hemoglobin, indicating that the adhesin domains seem to be particularly important for  P. gingivalis cells to agglutinate erythrocytes and bind hemoglobin, leading to heme acquisition.	bind
29728	4	8898	6	13	NULL	NULL	NULL	statement 2	Process		leads to					heme acquisition	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17955_s_11	10364243	A  rgpA kgp hagA triple mutant constructed in this study exhibited no hemagglutination using sheep erythrocytes or hemoglobin binding activity, as determined by a solid-phase binding assay with horseradish peroxidase-conjugated human hemoglobin, indicating that the adhesin domains seem to be particularly important for  P. gingivalis cells to agglutinate erythrocytes and bind hemoglobin, leading to heme acquisition.	bind
29729	5	8898	6	13	NULL	NULL	NULL	statement 3	Process		leads to					heme acquisition	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17955_s_11	10364243	A  rgpA kgp hagA triple mutant constructed in this study exhibited no hemagglutination using sheep erythrocytes or hemoglobin binding activity, as determined by a solid-phase binding assay with horseradish peroxidase-conjugated human hemoglobin, indicating that the adhesin domains seem to be particularly important for  P. gingivalis cells to agglutinate erythrocytes and bind hemoglobin, leading to heme acquisition.	bind
29730	6	8898	6	13	NULL	NULL	NULL				are important for			adhesion domain		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17955_s_11	10364243	A  rgpA kgp hagA triple mutant constructed in this study exhibited no hemagglutination using sheep erythrocytes or hemoglobin binding activity, as determined by a solid-phase binding assay with horseradish peroxidase-conjugated human hemoglobin, indicating that the adhesin domains seem to be particularly important for  P. gingivalis cells to agglutinate erythrocytes and bind hemoglobin, leading to heme acquisition.	bind
29731	7	8898	6	13	NULL	NULL	NULL				are important for			adhesion domain		statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17955_s_11	10364243	A  rgpA kgp hagA triple mutant constructed in this study exhibited no hemagglutination using sheep erythrocytes or hemoglobin binding activity, as determined by a solid-phase binding assay with horseradish peroxidase-conjugated human hemoglobin, indicating that the adhesin domains seem to be particularly important for  P. gingivalis cells to agglutinate erythrocytes and bind hemoglobin, leading to heme acquisition.	bind
47000	8	8898	6	13	NULL	NULL	NULL	rgpA kgp hagA	GP	triple mutant	does not exhibit					hemoglobin	GP	binding activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17955_s_11	10364243	A  rgpA kgp hagA triple mutant constructed in this study exhibited no hemagglutination using sheep erythrocytes or hemoglobin binding activity, as determined by a solid-phase binding assay with horseradish peroxidase-conjugated human hemoglobin, indicating that the adhesin domains seem to be particularly important for  P. gingivalis cells to agglutinate erythrocytes and bind hemoglobin, leading to heme acquisition.	bind
38437	1	8898	7	NULL	NULL	0	NULL	P. gingivalis cells	NULL		agglutinate	NULL				erythrocytes	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_25_17955_s_11	10364243	A  rgpA kgp hagA triple mutant constructed in this study exhibited no hemagglutination using sheep erythrocytes or hemoglobin binding activity, as determined by a solid-phase binding assay with horseradish peroxidase-conjugated human hemoglobin, indicating that the adhesin domains seem to be particularly important for  P. gingivalis cells to agglutinate erythrocytes and bind hemoglobin, leading to heme acquisition.	bind
38438	2	8898	7	NULL	NULL	0	NULL	P. gingivalis cells	NULL		bind	NULL				hemoglobin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_25_17955_s_11	10364243	A  rgpA kgp hagA triple mutant constructed in this study exhibited no hemagglutination using sheep erythrocytes or hemoglobin binding activity, as determined by a solid-phase binding assay with horseradish peroxidase-conjugated human hemoglobin, indicating that the adhesin domains seem to be particularly important for  P. gingivalis cells to agglutinate erythrocytes and bind hemoglobin, leading to heme acquisition.	bind
38439	3	8898	7	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				heme acquisition	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_25_17955_s_11	10364243	A  rgpA kgp hagA triple mutant constructed in this study exhibited no hemagglutination using sheep erythrocytes or hemoglobin binding activity, as determined by a solid-phase binding assay with horseradish peroxidase-conjugated human hemoglobin, indicating that the adhesin domains seem to be particularly important for  P. gingivalis cells to agglutinate erythrocytes and bind hemoglobin, leading to heme acquisition.	bind
38440	4	8898	7	NULL	NULL	0	NULL		NULL		is important for	NULL		adhesin domains		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_25_17955_s_11	10364243	A  rgpA kgp hagA triple mutant constructed in this study exhibited no hemagglutination using sheep erythrocytes or hemoglobin binding activity, as determined by a solid-phase binding assay with horseradish peroxidase-conjugated human hemoglobin, indicating that the adhesin domains seem to be particularly important for  P. gingivalis cells to agglutinate erythrocytes and bind hemoglobin, leading to heme acquisition.	bind
38441	5	8898	7	NULL	NULL	0	NULL		NULL		is important for	NULL		adhesin domains		statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_25_17955_s_11	10364243	A  rgpA kgp hagA triple mutant constructed in this study exhibited no hemagglutination using sheep erythrocytes or hemoglobin binding activity, as determined by a solid-phase binding assay with horseradish peroxidase-conjugated human hemoglobin, indicating that the adhesin domains seem to be particularly important for  P. gingivalis cells to agglutinate erythrocytes and bind hemoglobin, leading to heme acquisition.	bind
38504	6	8898	7	NULL	NULL	0	NULL	rgpA kgp hagA	NULL	triple mutant	does not exhibit	NULL				hemagglutination	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_25_17955_s_11	10364243	A  rgpA kgp hagA triple mutant constructed in this study exhibited no hemagglutination using sheep erythrocytes or hemoglobin binding activity, as determined by a solid-phase binding assay with horseradish peroxidase-conjugated human hemoglobin, indicating that the adhesin domains seem to be particularly important for  P. gingivalis cells to agglutinate erythrocytes and bind hemoglobin, leading to heme acquisition.	bind
38508	7	8898	7	10	NULL	0	NULL	rgpA kgp hagA	NULL	triple mutant	does not exhibit	NULL				hemoglobin	NULL	binding activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17955_s_11	10364243	A  rgpA kgp hagA triple mutant constructed in this study exhibited no hemagglutination using sheep erythrocytes or hemoglobin binding activity, as determined by a solid-phase binding assay with horseradish peroxidase-conjugated human hemoglobin, indicating that the adhesin domains seem to be particularly important for  P. gingivalis cells to agglutinate erythrocytes and bind hemoglobin, leading to heme acquisition.	bind
47001	8	8898	7	10	NULL	0	NULL	statement 1	NULL		leads to	NULL				heme acquisition 	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_25_17955_s_11	10364243	A  rgpA kgp hagA triple mutant constructed in this study exhibited no hemagglutination using sheep erythrocytes or hemoglobin binding activity, as determined by a solid-phase binding assay with horseradish peroxidase-conjugated human hemoglobin, indicating that the adhesin domains seem to be particularly important for  P. gingivalis cells to agglutinate erythrocytes and bind hemoglobin, leading to heme acquisition.	bind
29732	1	8900	6	13	NULL	NULL	NULL	tegument protein	GP		bind					VP1/2	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_j-virol_80_1_16352544_s_5	16352544	A  second tegument protein that binds to VP1/2, UL37, was necessary for wild-type  transport but was not essential for this process.	bind
29733	2	8900	6	13	NULL	NULL	NULL	tegument protein	GP		bind					UL37	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_j-virol_80_1_16352544_s_5	16352544	A  second tegument protein that binds to VP1/2, UL37, was necessary for wild-type  transport but was not essential for this process.	bind
29734	3	8900	6	13	NULL	NULL	NULL	statement 1	Process		is necessary for					transport	Process	wild type			NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_j-virol_80_1_16352544_s_5	16352544	A  second tegument protein that binds to VP1/2, UL37, was necessary for wild-type  transport but was not essential for this process.	bind
29735	4	8900	6	13	NULL	NULL	NULL	statement 2	Process		is necessary for					transport	Process	wild type			NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_j-virol_80_1_16352544_s_5	16352544	A  second tegument protein that binds to VP1/2, UL37, was necessary for wild-type  transport but was not essential for this process.	bind
38513	1	8900	7	NULL	NULL	0	NULL	tegument protein	NULL		binds to	NULL				VP1/2	NULL				NULL		0	NULL	NULL	NULL	abs-batch0550-0559_j-virol_80_1_16352544_s_5	16352544	A  second tegument protein that binds to VP1/2, UL37, was necessary for wild-type  transport but was not essential for this process.	bind
38514	2	8900	7	NULL	NULL	0	NULL	tegument protein	NULL		binds to	NULL				UL37	NULL				NULL		0	NULL	NULL	NULL	abs-batch0550-0559_j-virol_80_1_16352544_s_5	16352544	A  second tegument protein that binds to VP1/2, UL37, was necessary for wild-type  transport but was not essential for this process.	bind
38515	3	8900	7	10	NULL	0	NULL	statement 1	NULL		is necessary for	NULL				transport	NULL	wild-type			NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_j-virol_80_1_16352544_s_5	16352544	A  second tegument protein that binds to VP1/2, UL37, was necessary for wild-type  transport but was not essential for this process.	bind
38518	4	8900	7	10	NULL	0	NULL	statement 2	NULL		is necessary for	NULL				transport	NULL	wild-type			NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_j-virol_80_1_16352544_s_5	16352544	A  second tegument protein that binds to VP1/2, UL37, was necessary for wild-type  transport but was not essential for this process.	bind
29736	1	8901	6	13	NULL	NULL	NULL	synaptotagmin protein	GP		bind					trimeric SNARE complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_12_6567_s_96	8636067	A  second vesicle protein synaptotagmin can bind to the trimeric SNARE  complex, and there is compelling evidence that synaptotagmin acts as a  calcium-dependent regulator of transmitter release (reviewed by  Littleton and Bellen(1995)).	bind
29737	2	8901	6	13	NULL	NULL	NULL	synaptotagmin	GP		is a type of					second vesicle protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_12_6567_s_96	8636067	A  second vesicle protein synaptotagmin can bind to the trimeric SNARE  complex, and there is compelling evidence that synaptotagmin acts as a  calcium-dependent regulator of transmitter release (reviewed by  Littleton and Bellen(1995)).	bind
29738	3	8901	6	13	NULL	NULL	NULL	synaptotagmin	Process		acts as a 					transmitter release	GP	regulator of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_12_6567_s_96	8636067	A  second vesicle protein synaptotagmin can bind to the trimeric SNARE  complex, and there is compelling evidence that synaptotagmin acts as a  calcium-dependent regulator of transmitter release (reviewed by  Littleton and Bellen(1995)).	bind
29739	4	8901	6	13	NULL	NULL	NULL	statement 3	Process		is dependent on					calcium	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_12_6567_s_96	8636067	A  second vesicle protein synaptotagmin can bind to the trimeric SNARE  complex, and there is compelling evidence that synaptotagmin acts as a  calcium-dependent regulator of transmitter release (reviewed by  Littleton and Bellen(1995)).	bind
38528	1	8901	7	NULL	NULL	0	NULL	synaptotagmin	NULL		bind	NULL				trimeric SNARE complex	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_12_6567_s_96	8636067	A  second vesicle protein synaptotagmin can bind to the trimeric SNARE  complex, and there is compelling evidence that synaptotagmin acts as a  calcium-dependent regulator of transmitter release (reviewed by  Littleton and Bellen(1995)).	bind
38534	2	8901	7	10	NULL	0	NULL	synaptotagmin	NULL		acts as a	NULL				regulator release	NULL	regulator of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_12_6567_s_96	8636067	A  second vesicle protein synaptotagmin can bind to the trimeric SNARE  complex, and there is compelling evidence that synaptotagmin acts as a  calcium-dependent regulator of transmitter release (reviewed by  Littleton and Bellen(1995)).	bind
38544	3	8901	7	10	NULL	0	NULL	statement 2	NULL		is dependent on	NULL				calcium	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_12_6567_s_96	8636067	A  second vesicle protein synaptotagmin can bind to the trimeric SNARE  complex, and there is compelling evidence that synaptotagmin acts as a  calcium-dependent regulator of transmitter release (reviewed by  Littleton and Bellen(1995)).	bind
38550	4	8901	7	NULL	NULL	0	NULL	synaptotagmin	NULL		is a type of	NULL				second vesicle protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_12_6567_s_96	8636067	A  second vesicle protein synaptotagmin can bind to the trimeric SNARE  complex, and there is compelling evidence that synaptotagmin acts as a  calcium-dependent regulator of transmitter release (reviewed by  Littleton and Bellen(1995)).	bind
29740	1	8902	6	13	NULL	NULL	NULL	Ubiquitin	GP	binders of	is associated with					clathrin coat	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_j-biol-chem_281_31_16735510_s_6	16735510	A  set of clathrin coat-associated binders of ubiquitin also bind Nedd8,  but they undergo ubiquitylation, not neddylation.	bind
29741	2	8902	6	13	NULL	NULL	NULL	statement 1	GP		bind					Nedd8	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_j-biol-chem_281_31_16735510_s_6	16735510	A  set of clathrin coat-associated binders of ubiquitin also bind Nedd8,  but they undergo ubiquitylation, not neddylation.	bind
29742	3	8902	6	13	NULL	NULL	NULL	statement 1	GP		undergo					ubiquitylation	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_j-biol-chem_281_31_16735510_s_6	16735510	A  set of clathrin coat-associated binders of ubiquitin also bind Nedd8,  but they undergo ubiquitylation, not neddylation.	bind
29743	4	8902	6	13	NULL	NULL	NULL	statement 1	GP		does not undergo					neddylation	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_j-biol-chem_281_31_16735510_s_6	16735510	A  set of clathrin coat-associated binders of ubiquitin also bind Nedd8,  but they undergo ubiquitylation, not neddylation.	bind
38560	1	8902	7	10	NULL	0	NULL	Ubiquitin		binders of	is associated with					clathrin coat					NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_j-biol-chem_281_31_16735510_s_6	16735510	A  set of clathrin coat-associated binders of ubiquitin also bind Nedd8,  but they undergo ubiquitylation, not neddylation.	bind
38562	2	8902	7	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL				Nedd8	NULL				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_j-biol-chem_281_31_16735510_s_6	16735510	A  set of clathrin coat-associated binders of ubiquitin also bind Nedd8,  but they undergo ubiquitylation, not neddylation.	bind
38564	3	8902	7	10	NULL	0	NULL	statement 1			undergo					ubiquitylation					NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_j-biol-chem_281_31_16735510_s_6	16735510	A  set of clathrin coat-associated binders of ubiquitin also bind Nedd8,  but they undergo ubiquitylation, not neddylation.	bind
38567	4	8902	7	10	NULL	0	NULL	statement 1			does not undergo					neddylation					NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_j-biol-chem_281_31_16735510_s_6	16735510	A  set of clathrin coat-associated binders of ubiquitin also bind Nedd8,  but they undergo ubiquitylation, not neddylation.	bind
29744	1	8903	6	13	NULL	NULL	NULL	I-CRS peptide	GP		bind					SK-Hep cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_4_1807_s_132	7829517	A  shows the concentration  dependence of the binding of  I-CRS peptide ( sis)  to SK-Hep cells at pH 7.4.	bind
38568	1	8903	7	NULL	NULL	0	NULL	I-CRS peptide( sis)	NULL		bind	NULL				SK-Hep cells	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_4_1807_s_132	7829517	A  shows the concentration  dependence of the binding of  I-CRS peptide ( sis)  to SK-Hep cells at pH 7.4.	bind
29844	1	8904	6	13	NULL	NULL	NULL	C4b	GP		bind					LOS	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_51_50853_s_156	14525973	A  siaD galE mutant of strain MC58 (unencapsulated; Glc   HepI and 3-PEA on HepII ( LOS PEA+)) and its isogenic  lpt-3 mutant (lacking PEA on HepII ( LOS PEA-)) were incubated with NHS (the 500-mul reaction mixture contained 3 x 108 bacteria and NHS at a final concentration of 30%), and C4b binding to LOS was analyzed  as described in the legend to  Fig. 1.	bind
38597	1	8904	7	NULL	NULL	0	NULL	C4b 	NULL		bind	NULL				LOS	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_51_50853_s_156	14525973	A  siaD galE mutant of strain MC58 (unencapsulated; Glc   HepI and 3-PEA on HepII ( LOS PEA+)) and its isogenic  lpt-3 mutant (lacking PEA on HepII ( LOS PEA-)) were incubated with NHS (the 500-mul reaction mixture contained 3 x 108 bacteria and NHS at a final concentration of 30%), and C4b binding to LOS was analyzed  as described in the legend to  Fig. 1.	bind
29745	1	8905	6	13	NULL	NULL	NULL	BARD1	GP		bind					GST-BARD1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_104_5_743_s_193	11257228	A  significant amount of the input BARD1 and  BRCA1 bound to GST-BARD1 but not to  GST.	bind
29746	2	8905	6	13	NULL	NULL	NULL	BRCA1	GP		bind					GST-BARD1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_104_5_743_s_193	11257228	A  significant amount of the input BARD1 and  BRCA1 bound to GST-BARD1 but not to  GST.	bind
29747	3	8905	6	13	NULL	NULL	NULL	BARD1	GP		does not bind					GST	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_104_5_743_s_193	11257228	A  significant amount of the input BARD1 and  BRCA1 bound to GST-BARD1 but not to  GST.	bind
29748	4	8905	6	13	NULL	NULL	NULL	BRCA1	GP		does not bind					GST	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_104_5_743_s_193	11257228	A  significant amount of the input BARD1 and  BRCA1 bound to GST-BARD1 but not to  GST.	bind
38598	1	8905	7	NULL	NULL	0	NULL	BARD1	NULL		bind	NULL				GST-BARD1	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_104_5_743_s_193	11257228	A  significant amount of the input BARD1 and  BRCA1 bound to GST-BARD1 but not to  GST.	bind
38599	2	8905	7	NULL	NULL	0	NULL	BRCA1	NULL		bind	NULL				GST-BARD1	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_104_5_743_s_193	11257228	A  significant amount of the input BARD1 and  BRCA1 bound to GST-BARD1 but not to  GST.	bind
38600	3	8905	7	NULL	NULL	0	NULL	BARD1	NULL		does not bind	NULL				GST	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_104_5_743_s_193	11257228	A  significant amount of the input BARD1 and  BRCA1 bound to GST-BARD1 but not to  GST.	bind
38601	4	8905	7	NULL	NULL	0	NULL	 BRCA1	NULL		does not bind	NULL				GST	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_104_5_743_s_193	11257228	A  significant amount of the input BARD1 and  BRCA1 bound to GST-BARD1 but not to  GST.	bind
29749	1	8906	6	13	NULL	NULL	NULL	BDNF	GP		bind					trkB	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19669_s_89	7649974	A  similar  K   has also been determined for  BDNF binding to  trkB( 64) .	bind
38602	1	8906	7	NULL	NULL	0	NULL	BDNF 	NULL		bind	NULL				trkB	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_34_19669_s_89	7649974	A  similar  K   has also been determined for  BDNF binding to  trkB( 64) .	bind
29750	1	8907	6	13	NULL	NULL	NULL	IgG3	GP		bind					carbohydrate antigen	Chemical	multivalent			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_3_1527_s_146	8576148	A  similar finding was reported for IgG3 binding to a multivalent  carbohydrate antigen, and the effect was attributed to the tendency of  IgG3 to aggregate( 24) .	bind
29751	2	8907	6	13	NULL	NULL	NULL	statement 1	Process		contribute to					IgG3 	GP	aggregation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_3_1527_s_146	8576148	A  similar finding was reported for IgG3 binding to a multivalent  carbohydrate antigen, and the effect was attributed to the tendency of  IgG3 to aggregate( 24) .	bind
38603	1	8907	7	10	NULL	0	NULL	IgG3			bind					carbohydrate antigen		multivalent			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_3_1527_s_146	8576148	A  similar finding was reported for IgG3 binding to a multivalent  carbohydrate antigen, and the effect was attributed to the tendency of  IgG3 to aggregate( 24) .	bind
38604	2	8907	7	NULL	NULL	0	NULL	IgG3	NULL		tendency to	NULL				aggregate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_3_1527_s_146	8576148	A  similar finding was reported for IgG3 binding to a multivalent  carbohydrate antigen, and the effect was attributed to the tendency of  IgG3 to aggregate( 24) .	bind
38605	3	8907	7	10	NULL	0	NULL	statement 1	NULL		is attributed to	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_3_1527_s_146	8576148	A  similar finding was reported for IgG3 binding to a multivalent  carbohydrate antigen, and the effect was attributed to the tendency of  IgG3 to aggregate( 24) .	bind
29845	1	8908	6	13	NULL	NULL	NULL	HP1	GP		functions in					heterochromatin	Chromosome	assembly of			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_15_1823_s_146	12897052	A  similar function for HP1 in the assembly of heterochromatin has been proposed,  although dimerization of HP1 via the C-terminal chromo shadow domain makes the  binding of two histone tails from the same nucleosome, as well as separate  ones, possible.	bind
29846	2	8908	6	13	NULL	NULL	NULL	HP1	GP		bind			C-terminal chromo shadow domain		HP1	GP		C-terminal chromo shadow domain		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_15_1823_s_146	12897052	A  similar function for HP1 in the assembly of heterochromatin has been proposed,  although dimerization of HP1 via the C-terminal chromo shadow domain makes the  binding of two histone tails from the same nucleosome, as well as separate  ones, possible.	bind
29847	3	8908	6	13	NULL	NULL	NULL	histone tails	GP		bind					histone tails	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_15_1823_s_146	12897052	A  similar function for HP1 in the assembly of heterochromatin has been proposed,  although dimerization of HP1 via the C-terminal chromo shadow domain makes the  binding of two histone tails from the same nucleosome, as well as separate  ones, possible.	bind
29848	4	8908	6	13	NULL	NULL	NULL	statement 2	Process		allows					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_15_1823_s_146	12897052	A  similar function for HP1 in the assembly of heterochromatin has been proposed,  although dimerization of HP1 via the C-terminal chromo shadow domain makes the  binding of two histone tails from the same nucleosome, as well as separate  ones, possible.	bind
38606	1	8908	7	NULL	NULL	0	NULL	HP1	NULL		assembles	NULL				heterochromatin	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_17_15_1823_s_146	12897052	A  similar function for HP1 in the assembly of heterochromatin has been proposed,  although dimerization of HP1 via the C-terminal chromo shadow domain makes the  binding of two histone tails from the same nucleosome, as well as separate  ones, possible.	bind
38607	2	8908	7	10	NULL	0	NULL	HP1		dimerization of	occurs via					HP1			C-terminal chromo shadow domain		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_15_1823_s_146	12897052	A  similar function for HP1 in the assembly of heterochromatin has been proposed,  although dimerization of HP1 via the C-terminal chromo shadow domain makes the  binding of two histone tails from the same nucleosome, as well as separate  ones, possible.	bind
38608	3	8908	7	NULL	NULL	0	NULL	histone tails	NULL		bind	NULL				histone tails	NULL				NULL	nucleosome	0	NULL	NULL	NULL	gw60_genesdev_17_15_1823_s_146	12897052	A  similar function for HP1 in the assembly of heterochromatin has been proposed,  although dimerization of HP1 via the C-terminal chromo shadow domain makes the  binding of two histone tails from the same nucleosome, as well as separate  ones, possible.	bind
38609	4	8908	7	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_17_15_1823_s_146	12897052	A  similar function for HP1 in the assembly of heterochromatin has been proposed,  although dimerization of HP1 via the C-terminal chromo shadow domain makes the  binding of two histone tails from the same nucleosome, as well as separate  ones, possible.	bind
29752	1	8910	6	13	NULL	NULL	NULL	sin3	GP	mutations of	allows					HO	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4095_s_124	16705163	A  sin3 mutation also allows  HO to be expressed despite a  gcn5 mutation ( ) and raises the question of whether SWI/SNF binds to the  HO promoter in the  gcn5 sin3 strain.	bind
38614	1	8910	7	10	NULL	0	NULL	sin3	NULL	mutation of	allows	NULL				HO	NULL	expression of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4095_s_124	16705163	A  sin3 mutation also allows  HO to be expressed despite a  gcn5 mutation ( ) and raises the question of whether SWI/SNF binds to the  HO promoter in the  gcn5 sin3 strain.	bind
38615	2	8910	7	10	NULL	0	NULL	statement 2	NULL		occurs despite	NULL				gcn5	NULL	mutation of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4095_s_124	16705163	A  sin3 mutation also allows  HO to be expressed despite a  gcn5 mutation ( ) and raises the question of whether SWI/SNF binds to the  HO promoter in the  gcn5 sin3 strain.	bind
29753	1	8911	6	13	NULL	NULL	NULL	Aprataxin	GP		bind					DNA molecule	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_20_13939_s_129	16547001	A  single asterisk indicates unbound DNA,  two asterisks indicate the Aprataxin-DNA complex, and  three asterisks indicate more than one molecule of Aprataxin binding to one DNA molecule.	bind
38616	1	8911	7	NULL	NULL	0	NULL	Aprataxin	NULL		bind	NULL				DNA molecule	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_20_13939_s_129	16547001	A  single asterisk indicates unbound DNA,  two asterisks indicate the Aprataxin-DNA complex, and  three asterisks indicate more than one molecule of Aprataxin binding to one DNA molecule.	bind
29754	1	8912	6	13	NULL	NULL	NULL	p65	GP		bind					PPR	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_26_23570_s_174	12684509	A  small increase in p65 binding to the PPR was also detected.	bind
38617	1	8912	7	NULL	NULL	0	NULL	p65	NULL		bind	NULL				PPR	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_26_23570_s_174	12684509	A  small increase in p65 binding to the PPR was also detected.	bind
29755	1	8913	6	13	NULL	NULL	NULL	MAP4	GP		bind		directly	proline-rich region in the C-terminal half		Sept 2:6:7 heterotrimer	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_mol-biol-cell_16_10_16093351_s_6	16093351	A  small, proline-rich region in the C-terminal half of MAP4 bound directly  to a Sept 2:6:7 heterotrimer, and to the Sept2 monomer.	bind
29756	2	8913	6	13	NULL	NULL	NULL	MAP4	GP		bind		directly	proline-rich region in the C-terminal half		Sept2 monomer	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_mol-biol-cell_16_10_16093351_s_6	16093351	A  small, proline-rich region in the C-terminal half of MAP4 bound directly  to a Sept 2:6:7 heterotrimer, and to the Sept2 monomer.	bind
38618	1	8913	7	NULL	NULL	0	NULL	MAP4	NULL		bind	NULL	directly	proline-rich region in the C-terminal half		Sept 2:6:7 heterotrimer	NULL				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_mol-biol-cell_16_10_16093351_s_6	16093351	A  small, proline-rich region in the C-terminal half of MAP4 bound directly  to a Sept 2:6:7 heterotrimer, and to the Sept2 monomer.	bind
38619	2	8913	7	NULL	NULL	0	NULL	MAP4	NULL		bind	NULL	directly	proline-rich region in the C-terminal half		Sept2 monomer	NULL				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_mol-biol-cell_16_10_16093351_s_6	16093351	A  small, proline-rich region in the C-terminal half of MAP4 bound directly  to a Sept 2:6:7 heterotrimer, and to the Sept2 monomer.	bind
29757	1	8914	6	13	NULL	NULL	NULL	cholecystokinin-releasing peptide	GP		bind		specifically			small-intestinal cells	Cell	rat;;isolated			NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_59_0_221_s_857	9074762	A  specific binding of the cholecystokinin-releasing peptide (monitor peptide) to isolated  rat small-intestinal cells.	bind
29758	2	8914	6	13	NULL	NULL	NULL	cholecystokinin-releasing peptide	GP		is					monitor peptide	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_59_0_221_s_857	9074762	A  specific binding of the cholecystokinin-releasing peptide (monitor peptide) to isolated  rat small-intestinal cells.	bind
38620	1	8914	7	10	NULL	0	NULL	cholecystokinin-releasing peptide			bind		specifically			small-intestinal cells		isolated;;rat			NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_59_0_221_s_857	9074762	A  specific binding of the cholecystokinin-releasing peptide (monitor peptide) to isolated  rat small-intestinal cells.	bind
38621	2	8914	7	NULL	NULL	0	NULL	cholecystokinin-releasing peptide	NULL		is	NULL				monitor peptide	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevphysiol_59_0_221_s_857	9074762	A  specific binding of the cholecystokinin-releasing peptide (monitor peptide) to isolated  rat small-intestinal cells.	bind
29759	1	8916	6	13	NULL	NULL	NULL	influenza C virus	Organism		bind		preferentially			single cell surface glycoprotein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_30_17815_s_294	7629082	A  surprising finding of our work was that influenza C virus  preferentially binds to a single cell surface glycoprotein.	bind
38622	1	8916	7	NULL	NULL	0	NULL	influenza C virus 	NULL		binds	NULL	preferentially			single cell surface glycoprotein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_30_17815_s_294	7629082	A  surprising finding of our work was that influenza C virus  preferentially binds to a single cell surface glycoprotein.	bind
29760	1	8917	6	13	NULL	NULL	NULL	oppA	GP	T. denticola;; mutant	bind					plasminogen	GP	reduced amount of;;soluble			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_4_1884_s_11	10722578	A  T. denticola oppA mutant bound reduced amounts of soluble plasminogen, and plasminogen binding to the parent strain was inhibited by the lysine analog  -aminocaproic acid.	bind
29761	2	8917	6	13	NULL	NULL	NULL	plasminogen	GP		bind					oppA	GP	T. denticola			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_4_1884_s_11	10722578	A  T. denticola oppA mutant bound reduced amounts of soluble plasminogen, and plasminogen binding to the parent strain was inhibited by the lysine analog  -aminocaproic acid.	bind
29762	3	8917	6	13	NULL	NULL	NULL	statement 2	Process		is inhibited by					aminocaproic acid	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_4_1884_s_11	10722578	A  T. denticola oppA mutant bound reduced amounts of soluble plasminogen, and plasminogen binding to the parent strain was inhibited by the lysine analog  -aminocaproic acid.	bind
47008	4	8917	6	13	NULL	NULL	NULL	aminocaproic acid	Chemical		is a type of					lysine analog	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_4_1884_s_11	10722578	A  T. denticola oppA mutant bound reduced amounts of soluble plasminogen, and plasminogen binding to the parent strain was inhibited by the lysine analog  -aminocaproic acid.	bind
38623	1	8917	7	10	NULL	0	NULL	oppA	NULL	T. denticola;;mutant	bind	NULL				plasminogen	NULL	reduced amount of;;soluble			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_4_1884_s_11	10722578	A  T. denticola oppA mutant bound reduced amounts of soluble plasminogen, and plasminogen binding to the parent strain was inhibited by the lysine analog  -aminocaproic acid.	bind
38624	2	8917	7	10	NULL	0	NULL	plasminogen	NULL		bind	NULL				oppA	NULL	T. denticola			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_4_1884_s_11	10722578	A  T. denticola oppA mutant bound reduced amounts of soluble plasminogen, and plasminogen binding to the parent strain was inhibited by the lysine analog  -aminocaproic acid.	bind
38625	3	8917	7	NULL	NULL	0	NULL	aminocaproic acid	NULL		inhibits	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_4_1884_s_11	10722578	A  T. denticola oppA mutant bound reduced amounts of soluble plasminogen, and plasminogen binding to the parent strain was inhibited by the lysine analog  -aminocaproic acid.	bind
38626	4	8917	7	NULL	NULL	0	NULL	aminocaproic acid	NULL		is a type of	NULL				lysine analog	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_4_1884_s_11	10722578	A  T. denticola oppA mutant bound reduced amounts of soluble plasminogen, and plasminogen binding to the parent strain was inhibited by the lysine analog  -aminocaproic acid.	bind
29763	1	8918	6	13	NULL	NULL	NULL	secretion substrate	GP		bind			amino acid region		secretion chaperone 	GP	putative			NULL		NULL	NULL	NULL	NULL	gw60_cell_102_4_487_s_272	10966110	A  third would be the amino acid region of the secretion substrate bound  by its cognate putative secretion chaperone (translational regulator) and held at the base  of the secretion apparatus until secretion can occur.	bind
29764	2	8918	6	13	NULL	NULL	NULL	secretion chaperone	GP		is a type of					translational regulator	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_102_4_487_s_272	10966110	A  third would be the amino acid region of the secretion substrate bound  by its cognate putative secretion chaperone (translational regulator) and held at the base  of the secretion apparatus until secretion can occur.	bind
38627	1	8918	7	10	NULL	0	NULL	secretion chaperone	NULL	cognate putative	bind	NULL				secretion substrate	NULL		amino acid region of		NULL		NULL	NULL	NULL	NULL	gw60_cell_102_4_487_s_272	10966110	A  third would be the amino acid region of the secretion substrate bound  by its cognate putative secretion chaperone (translational regulator) and held at the base  of the secretion apparatus until secretion can occur.	bind
38628	2	8918	7	10	NULL	0	NULL	secretion chaperone	NULL		is a type of	NULL				translational regulator	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cell_102_4_487_s_272	10966110	A  third would be the amino acid region of the secretion substrate bound  by its cognate putative secretion chaperone (translational regulator) and held at the base  of the secretion apparatus until secretion can occur.	bind
29765	1	8919	6	13	NULL	NULL	NULL	v-Crk	GP		bind					paxillin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31219_s_101	8537387	A  titration experiment showed that half maximal binding was observed at  around 10-20 nM  of the GST-Csk SH3/2 protein ( Fig. 4 A), an affinity that is severalfold weaker than that  of v-Crk binding to paxillin.	bind
47011	2	8919	6	13	NULL	NULL	NULL	GST-Csk SH3/2 protein	GP		bind					paxillin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31219_s_101	8537387	A  titration experiment showed that half maximal binding was observed at  around 10-20 nM  of the GST-Csk SH3/2 protein ( Fig. 4 A), an affinity that is severalfold weaker than that  of v-Crk binding to paxillin.	bind
47012	3	8919	6	13	NULL	NULL	NULL	statement 2	Process	affinity of	is weaker than					statement 1	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31219_s_101	8537387	A  titration experiment showed that half maximal binding was observed at  around 10-20 nM  of the GST-Csk SH3/2 protein ( Fig. 4 A), an affinity that is severalfold weaker than that  of v-Crk binding to paxillin.	bind
38629	1	8919	7	NULL	NULL	0	NULL	v-Crk 	NULL		bind	NULL				paxillin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31219_s_101	8537387	A  titration experiment showed that half maximal binding was observed at  around 10-20 nM  of the GST-Csk SH3/2 protein ( Fig. 4 A), an affinity that is severalfold weaker than that  of v-Crk binding to paxillin.	bind
38630	2	8919	7	NULL	NULL	0	NULL	GST-Csk SH3/2 protein	NULL		bind	NULL				paxillin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31219_s_101	8537387	A  titration experiment showed that half maximal binding was observed at  around 10-20 nM  of the GST-Csk SH3/2 protein ( Fig. 4 A), an affinity that is severalfold weaker than that  of v-Crk binding to paxillin.	bind
38631	3	8919	7	NULL	NULL	0	NULL	statement 2	NULL	affinity of	is weaker than	NULL				statement 1	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31219_s_101	8537387	A  titration experiment showed that half maximal binding was observed at  around 10-20 nM  of the GST-Csk SH3/2 protein ( Fig. 4 A), an affinity that is severalfold weaker than that  of v-Crk binding to paxillin.	bind
29766	1	8920	6	13	NULL	NULL	NULL	Tax	GP		is a type of					transactivator	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4450_s_680	12052856	A  trans-activator Tax of human T-cell leukemia virus type 1 binds to NF-kappa B p50 and serum response factor (SRF) and associates with enhancer DNAs of the NF-kappa B site and CArG box.	bind
29767	2	8920	6	13	NULL	NULL	NULL	Tax	GP	human T-cell leukemia virus type 1	bind					NF-kappaB p50	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4450_s_680	12052856	A  trans-activator Tax of human T-cell leukemia virus type 1 binds to NF-kappa B p50 and serum response factor (SRF) and associates with enhancer DNAs of the NF-kappa B site and CArG box.	bind
29768	3	8920	6	13	NULL	NULL	NULL	Tax	GP	human T-cell leukemia virus type 1	bind					SRF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4450_s_680	12052856	A  trans-activator Tax of human T-cell leukemia virus type 1 binds to NF-kappa B p50 and serum response factor (SRF) and associates with enhancer DNAs of the NF-kappa B site and CArG box.	bind
29769	4	8920	6	13	NULL	NULL	NULL	SRF	GP		is 					serum response factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4450_s_680	12052856	A  trans-activator Tax of human T-cell leukemia virus type 1 binds to NF-kappa B p50 and serum response factor (SRF) and associates with enhancer DNAs of the NF-kappa B site and CArG box.	bind
29770	5	8920	6	13	NULL	NULL	NULL	Tax	GP	human T-cell leukemia virus type 1	associates with					DNA	NucleicAcid			NF-kappaB binding site of enhancer	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4450_s_680	12052856	A  trans-activator Tax of human T-cell leukemia virus type 1 binds to NF-kappa B p50 and serum response factor (SRF) and associates with enhancer DNAs of the NF-kappa B site and CArG box.	bind
29771	6	8920	6	13	NULL	NULL	NULL	Tax	GP	human T-cell leukemia virus type 1	bind					DNA	NucleicAcid			CArG box of enhancer	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4450_s_680	12052856	A  trans-activator Tax of human T-cell leukemia virus type 1 binds to NF-kappa B p50 and serum response factor (SRF) and associates with enhancer DNAs of the NF-kappa B site and CArG box.	bind
38632	1	8920	7	NULL	NULL	0	NULL	Tax 	NULL	human T-cell leukemia virus type 1	binds to	NULL				NF-kappa B p50	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_13_4450_s_680	12052856	A  trans-activator Tax of human T-cell leukemia virus type 1 binds to NF-kappa B p50 and serum response factor (SRF) and associates with enhancer DNAs of the NF-kappa B site and CArG box.	bind
38633	2	8920	7	NULL	NULL	0	NULL	Tax	NULL	human T-cell leukemia virus type 1 	binds to	NULL				SRF	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_13_4450_s_680	12052856	A  trans-activator Tax of human T-cell leukemia virus type 1 binds to NF-kappa B p50 and serum response factor (SRF) and associates with enhancer DNAs of the NF-kappa B site and CArG box.	bind
38634	3	8920	7	10	NULL	0	NULL	Tax	NULL	human T-cell leukemia virus type 1	associate with	NULL				DNA	NULL			NF-kappa B site of enhancer	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4450_s_680	12052856	A  trans-activator Tax of human T-cell leukemia virus type 1 binds to NF-kappa B p50 and serum response factor (SRF) and associates with enhancer DNAs of the NF-kappa B site and CArG box.	bind
38635	4	8920	7	10	NULL	0	NULL	Tax	NULL	human T-cell leukemia virus type 1	associate with	NULL				DNA	NULL			CArG box of enhancer	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4450_s_680	12052856	A  trans-activator Tax of human T-cell leukemia virus type 1 binds to NF-kappa B p50 and serum response factor (SRF) and associates with enhancer DNAs of the NF-kappa B site and CArG box.	bind
38636	5	8920	7	NULL	NULL	0	NULL	SRF	NULL		is	NULL				serum response factor	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_13_4450_s_680	12052856	A  trans-activator Tax of human T-cell leukemia virus type 1 binds to NF-kappa B p50 and serum response factor (SRF) and associates with enhancer DNAs of the NF-kappa B site and CArG box.	bind
38637	6	8920	7	NULL	NULL	0	NULL	Tax	NULL		is a type of	NULL				trans-activator	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_13_4450_s_680	12052856	A  trans-activator Tax of human T-cell leukemia virus type 1 binds to NF-kappa B p50 and serum response factor (SRF) and associates with enhancer DNAs of the NF-kappa B site and CArG box.	bind
29772	1	8921	6	13	NULL	NULL	NULL	GST-p65 -beta-delta3	GP	truncated	bind		strongly			Cdc42	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_49_29071_s_66	7493928	A  truncated p65 -beta  construct,  GST-p65 -beta-delta3, continued to show strong Cdc42  binding, although binding to Rac was reduced ( Fig. 1).	bind
29773	2	8921	6	13	NULL	NULL	NULL	GST-p65 -beta-delta3	GP		bind		redduced			Rac	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_49_29071_s_66	7493928	A  truncated p65 -beta  construct,  GST-p65 -beta-delta3, continued to show strong Cdc42  binding, although binding to Rac was reduced ( Fig. 1).	bind
38671	1	8921	7	NULL	NULL	0	NULL	GST-p65 -beta-delta3	NULL		bind	NULL	strongly			Cdc42	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_49_29071_s_66	7493928	A  truncated p65 -beta  construct,  GST-p65 -beta-delta3, continued to show strong Cdc42  binding, although binding to Rac was reduced ( Fig. 1).	bind
38672	2	8921	7	NULL	NULL	0	NULL	GST-p65 -beta-delta3	NULL		bind	NULL	reduced			Rac	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_49_29071_s_66	7493928	A  truncated p65 -beta  construct,  GST-p65 -beta-delta3, continued to show strong Cdc42  binding, although binding to Rac was reduced ( Fig. 1).	bind
38673	3	8921	7	NULL	NULL	0	NULL	GST-p65 -beta-delta3	NULL		is a type of	NULL				truncated p65 -beta construct	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_49_29071_s_66	7493928	A  truncated p65 -beta  construct,  GST-p65 -beta-delta3, continued to show strong Cdc42  binding, although binding to Rac was reduced ( Fig. 1).	bind
29774	1	8922	6	13	NULL	NULL	NULL	UspA1 protein	GP		bind					MAb 17C7	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_4_2400_s_207	15784586	A  uspA1 mutant of MC317 (MC317.1) was constructed for use in this assay to eliminate expression of the UspA1 protein which also binds MAb 17C7.	bind
29775	2	8922	6	13	NULL	NULL	NULL	MC317.1	GP		is					uspA1 mutant of MC317	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_4_2400_s_207	15784586	A  uspA1 mutant of MC317 (MC317.1) was constructed for use in this assay to eliminate expression of the UspA1 protein which also binds MAb 17C7.	bind
29776	3	8922	6	13	NULL	NULL	NULL	statement 2	GP		eliminates					UspA1 protein	GP	expression of 			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_4_2400_s_207	15784586	A  uspA1 mutant of MC317 (MC317.1) was constructed for use in this assay to eliminate expression of the UspA1 protein which also binds MAb 17C7.	bind
38674	1	8922	7	NULL	NULL	0	NULL	UspA1 protein	NULL		binds to	NULL				MAb 17C7	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_73_4_2400_s_207	15784586	A  uspA1 mutant of MC317 (MC317.1) was constructed for use in this assay to eliminate expression of the UspA1 protein which also binds MAb 17C7.	bind
47018	2	8922	7	10	NULL	0	NULL	MC317.1	NULL		is	NULL				uspA1 mutant of MC317	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_73_4_2400_s_207	15784586	A  uspA1 mutant of MC317 (MC317.1) was constructed for use in this assay to eliminate expression of the UspA1 protein which also binds MAb 17C7.	bind
47019	3	8922	7	10	NULL	0	NULL	statement 2	NULL		eliminates	NULL				UspA1 protein	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_infectimmun_73_4_2400_s_207	15784586	A  uspA1 mutant of MC317 (MC317.1) was constructed for use in this assay to eliminate expression of the UspA1 protein which also binds MAb 17C7.	bind
29777	1	8923	6	13	NULL	NULL	NULL	PA26	GP	Xenopus	is homologous to					p53-activated gene	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_development_130_17_4161_s_502	12874135	A  Xenopus homolog of a human p53-activated gene,  PA26, is specifically expressed in the notochord.	bind
29778	2	8923	6	13	NULL	NULL	NULL	PA26	GP		is expressed in		specifically			notochord	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_development_130_17_4161_s_502	12874135	A  Xenopus homolog of a human p53-activated gene,  PA26, is specifically expressed in the notochord.	bind
38675	1	8923	7	10	NULL	0	NULL	PA26	NULL	Xenopus	is homologous to	NULL				 p53-activated gene	NULL	 human			NULL		NULL	NULL	NULL	NULL	gw60_development_130_17_4161_s_502	12874135	A  Xenopus homolog of a human p53-activated gene,  PA26, is specifically expressed in the notochord.	bind
38676	2	8923	7	NULL	NULL	0	NULL	PA26	NULL		is expressed in	NULL	specifically			notochord	NULL				NULL		0	NULL	NULL	NULL	gw60_development_130_17_4161_s_502	12874135	A  Xenopus homolog of a human p53-activated gene,  PA26, is specifically expressed in the notochord.	bind
29779	1	8924	6	13	NULL	NULL	NULL	MP90	GP		is a type of					mitotic phosphoprotein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_6_3257_s_3	9920862	A  Xenopus mitotic phosphoprotein, MP90, is very similar to an abundant mammalian nerve terminal protein, epsin, which binds the Eps15 homology (EH) domain of Eps15 and the alpha-adaptin subunit of the clathrin adaptor AP-2.	bind
29780	2	8924	6	13	NULL	NULL	NULL	MP90	GP	Xenopus	is similar to					epsin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_6_3257_s_3	9920862	A  Xenopus mitotic phosphoprotein, MP90, is very similar to an abundant mammalian nerve terminal protein, epsin, which binds the Eps15 homology (EH) domain of Eps15 and the alpha-adaptin subunit of the clathrin adaptor AP-2.	bind
29781	3	8924	6	13	NULL	NULL	NULL	epsin	GP		is a type of					mammalian nerve terminal protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_6_3257_s_3	9920862	A  Xenopus mitotic phosphoprotein, MP90, is very similar to an abundant mammalian nerve terminal protein, epsin, which binds the Eps15 homology (EH) domain of Eps15 and the alpha-adaptin subunit of the clathrin adaptor AP-2.	bind
29782	4	8924	6	13	NULL	NULL	NULL	epsin	GP		bind					Eps15	GP		EH domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_6_3257_s_3	9920862	A  Xenopus mitotic phosphoprotein, MP90, is very similar to an abundant mammalian nerve terminal protein, epsin, which binds the Eps15 homology (EH) domain of Eps15 and the alpha-adaptin subunit of the clathrin adaptor AP-2.	bind
29783	5	8924	6	13	NULL	NULL	NULL	Eps15 homology domain 	GP		is					EH domain	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_6_3257_s_3	9920862	A  Xenopus mitotic phosphoprotein, MP90, is very similar to an abundant mammalian nerve terminal protein, epsin, which binds the Eps15 homology (EH) domain of Eps15 and the alpha-adaptin subunit of the clathrin adaptor AP-2.	bind
29784	6	8924	6	13	NULL	NULL	NULL	epsin	GP		bind					AP-2	GP		alpha-adaptin subunit		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_6_3257_s_3	9920862	A  Xenopus mitotic phosphoprotein, MP90, is very similar to an abundant mammalian nerve terminal protein, epsin, which binds the Eps15 homology (EH) domain of Eps15 and the alpha-adaptin subunit of the clathrin adaptor AP-2.	bind
29785	7	8924	6	13	NULL	NULL	NULL	AP-2	GP		is a type of					clathrin adaptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_6_3257_s_3	9920862	A  Xenopus mitotic phosphoprotein, MP90, is very similar to an abundant mammalian nerve terminal protein, epsin, which binds the Eps15 homology (EH) domain of Eps15 and the alpha-adaptin subunit of the clathrin adaptor AP-2.	bind
38677	1	8924	7	10	NULL	0	NULL	MP90	NULL	Xenopus	is similar to	NULL				epsin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_6_3257_s_3	9920862	A  Xenopus mitotic phosphoprotein, MP90, is very similar to an abundant mammalian nerve terminal protein, epsin, which binds the Eps15 homology (EH) domain of Eps15 and the alpha-adaptin subunit of the clathrin adaptor AP-2.	bind
38678	2	8924	7	NULL	NULL	0	NULL	epsin	NULL		bind	NULL				Eps15	NULL		EH domain 		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_6_3257_s_3	9920862	A  Xenopus mitotic phosphoprotein, MP90, is very similar to an abundant mammalian nerve terminal protein, epsin, which binds the Eps15 homology (EH) domain of Eps15 and the alpha-adaptin subunit of the clathrin adaptor AP-2.	bind
38679	3	8924	7	NULL	NULL	0	NULL	epsin	NULL		bind	NULL				 AP-2	NULL		alpha-adaptin subunit 		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_6_3257_s_3	9920862	A  Xenopus mitotic phosphoprotein, MP90, is very similar to an abundant mammalian nerve terminal protein, epsin, which binds the Eps15 homology (EH) domain of Eps15 and the alpha-adaptin subunit of the clathrin adaptor AP-2.	bind
38680	4	8924	7	10	NULL	0	NULL	MP90	NULL		is a type of	NULL				mitotic phosphoprotein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_6_3257_s_3	9920862	A  Xenopus mitotic phosphoprotein, MP90, is very similar to an abundant mammalian nerve terminal protein, epsin, which binds the Eps15 homology (EH) domain of Eps15 and the alpha-adaptin subunit of the clathrin adaptor AP-2.	bind
38681	5	8924	7	10	NULL	0	NULL	epsin	NULL		is a type of	NULL				mammalian nerve terminal protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_6_3257_s_3	9920862	A  Xenopus mitotic phosphoprotein, MP90, is very similar to an abundant mammalian nerve terminal protein, epsin, which binds the Eps15 homology (EH) domain of Eps15 and the alpha-adaptin subunit of the clathrin adaptor AP-2.	bind
38682	6	8924	7	NULL	NULL	0	NULL	EH domain	NULL		is	NULL				Eps15 homology domain	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_6_3257_s_3	9920862	A  Xenopus mitotic phosphoprotein, MP90, is very similar to an abundant mammalian nerve terminal protein, epsin, which binds the Eps15 homology (EH) domain of Eps15 and the alpha-adaptin subunit of the clathrin adaptor AP-2.	bind
38683	7	8924	7	NULL	NULL	0	NULL	AP-2	NULL		is a type of	NULL				clathrin adaptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_6_3257_s_3	9920862	A  Xenopus mitotic phosphoprotein, MP90, is very similar to an abundant mammalian nerve terminal protein, epsin, which binds the Eps15 homology (EH) domain of Eps15 and the alpha-adaptin subunit of the clathrin adaptor AP-2.	bind
29786	1	8926	6	13	NULL	NULL	NULL	HBV	Organism		bind					HDL	GP				NULL		NULL	NULL	NULL	NULL	gw60_neurobiolaging_20_4_457_s_139	10604441	A "`hitchhiker"` method of cell entry has been suggested also for hepatitis B virus (HBV) bound to HDL or chylomicrons (this binding being mediated by apolipoprotein H), with the HBV-LP complex binding to hepatocytes via the LDL receptor (LDLR) or the LDLR-related protein/ 2-macroglogulin receptor (LRP) [  60].	bind
29787	2	8926	6	13	NULL	NULL	NULL	HBV	Organism		is					hepatitis B virus	Organism				NULL		NULL	NULL	NULL	NULL	gw60_neurobiolaging_20_4_457_s_139	10604441	A "`hitchhiker"` method of cell entry has been suggested also for hepatitis B virus (HBV) bound to HDL or chylomicrons (this binding being mediated by apolipoprotein H), with the HBV-LP complex binding to hepatocytes via the LDL receptor (LDLR) or the LDLR-related protein/ 2-macroglogulin receptor (LRP) [  60].	bind
29788	3	8926	6	13	NULL	NULL	NULL	HBV	Organism		bind					chylomicrons	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neurobiolaging_20_4_457_s_139	10604441	A "`hitchhiker"` method of cell entry has been suggested also for hepatitis B virus (HBV) bound to HDL or chylomicrons (this binding being mediated by apolipoprotein H), with the HBV-LP complex binding to hepatocytes via the LDL receptor (LDLR) or the LDLR-related protein/ 2-macroglogulin receptor (LRP) [  60].	bind
29789	4	8926	6	13	NULL	NULL	NULL	statement 3	Process		is mediated by					apolipoprotein H	GP				NULL		NULL	NULL	NULL	NULL	gw60_neurobiolaging_20_4_457_s_139	10604441	A "`hitchhiker"` method of cell entry has been suggested also for hepatitis B virus (HBV) bound to HDL or chylomicrons (this binding being mediated by apolipoprotein H), with the HBV-LP complex binding to hepatocytes via the LDL receptor (LDLR) or the LDLR-related protein/ 2-macroglogulin receptor (LRP) [  60].	bind
29790	5	8926	6	13	NULL	NULL	NULL	HBV-LP complex	Organism		bind					hepatocytes	Cell				NULL		NULL	NULL	NULL	NULL	gw60_neurobiolaging_20_4_457_s_139	10604441	A "`hitchhiker"` method of cell entry has been suggested also for hepatitis B virus (HBV) bound to HDL or chylomicrons (this binding being mediated by apolipoprotein H), with the HBV-LP complex binding to hepatocytes via the LDL receptor (LDLR) or the LDLR-related protein/ 2-macroglogulin receptor (LRP) [  60].	bind
29791	6	8926	6	13	NULL	NULL	NULL	statement 5	Process		occurs via					LDLR	GP				NULL		NULL	NULL	NULL	NULL	gw60_neurobiolaging_20_4_457_s_139	10604441	A "`hitchhiker"` method of cell entry has been suggested also for hepatitis B virus (HBV) bound to HDL or chylomicrons (this binding being mediated by apolipoprotein H), with the HBV-LP complex binding to hepatocytes via the LDL receptor (LDLR) or the LDLR-related protein/ 2-macroglogulin receptor (LRP) [  60].	bind
29792	7	8926	6	13	NULL	NULL	NULL	LRP	GP		is					LDLR-related protein/ 2-macroglogulin receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_neurobiolaging_20_4_457_s_139	10604441	A "`hitchhiker"` method of cell entry has been suggested also for hepatitis B virus (HBV) bound to HDL or chylomicrons (this binding being mediated by apolipoprotein H), with the HBV-LP complex binding to hepatocytes via the LDL receptor (LDLR) or the LDLR-related protein/ 2-macroglogulin receptor (LRP) [  60].	bind
29793	8	8926	6	13	NULL	NULL	NULL	statement 5	Process		occurs via					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_neurobiolaging_20_4_457_s_139	10604441	A "`hitchhiker"` method of cell entry has been suggested also for hepatitis B virus (HBV) bound to HDL or chylomicrons (this binding being mediated by apolipoprotein H), with the HBV-LP complex binding to hepatocytes via the LDL receptor (LDLR) or the LDLR-related protein/ 2-macroglogulin receptor (LRP) [  60].	bind
47028	9	8926	6	13	NULL	NULL	NULL	LDLR	GP		is					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_neurobiolaging_20_4_457_s_139	10604441	A "`hitchhiker"` method of cell entry has been suggested also for hepatitis B virus (HBV) bound to HDL or chylomicrons (this binding being mediated by apolipoprotein H), with the HBV-LP complex binding to hepatocytes via the LDL receptor (LDLR) or the LDLR-related protein/ 2-macroglogulin receptor (LRP) [  60].	bind
47029	10	8926	6	13	NULL	NULL	NULL	statement 6	Process		is an alternative to					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_neurobiolaging_20_4_457_s_139	10604441	A "`hitchhiker"` method of cell entry has been suggested also for hepatitis B virus (HBV) bound to HDL or chylomicrons (this binding being mediated by apolipoprotein H), with the HBV-LP complex binding to hepatocytes via the LDL receptor (LDLR) or the LDLR-related protein/ 2-macroglogulin receptor (LRP) [  60].	bind
47030	11	8926	6	13	NULL	NULL	NULL	2-macroglogulin receptor	GP		is a synonym of					LRP	GP				NULL		NULL	NULL	NULL	NULL	gw60_neurobiolaging_20_4_457_s_139	10604441	A "`hitchhiker"` method of cell entry has been suggested also for hepatitis B virus (HBV) bound to HDL or chylomicrons (this binding being mediated by apolipoprotein H), with the HBV-LP complex binding to hepatocytes via the LDL receptor (LDLR) or the LDLR-related protein/ 2-macroglogulin receptor (LRP) [  60].	bind
47032	12	8926	6	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_neurobiolaging_20_4_457_s_139	10604441	A "`hitchhiker"` method of cell entry has been suggested also for hepatitis B virus (HBV) bound to HDL or chylomicrons (this binding being mediated by apolipoprotein H), with the HBV-LP complex binding to hepatocytes via the LDL receptor (LDLR) or the LDLR-related protein/ 2-macroglogulin receptor (LRP) [  60].	bind
38686	1	8926	7	NULL	NULL	0	NULL	HBV	NULL		bind	NULL				HDL	NULL				NULL		0	NULL	NULL	NULL	gw60_neurobiolaging_20_4_457_s_139	10604441	A "`hitchhiker"` method of cell entry has been suggested also for hepatitis B virus (HBV) bound to HDL or chylomicrons (this binding being mediated by apolipoprotein H), with the HBV-LP complex binding to hepatocytes via the LDL receptor (LDLR) or the LDLR-related protein/ 2-macroglogulin receptor (LRP) [  60].	bind
38687	2	8926	7	NULL	NULL	0	NULL	HBV	NULL		bind	NULL				chylomicrons	NULL				NULL		0	NULL	NULL	NULL	gw60_neurobiolaging_20_4_457_s_139	10604441	A "`hitchhiker"` method of cell entry has been suggested also for hepatitis B virus (HBV) bound to HDL or chylomicrons (this binding being mediated by apolipoprotein H), with the HBV-LP complex binding to hepatocytes via the LDL receptor (LDLR) or the LDLR-related protein/ 2-macroglogulin receptor (LRP) [  60].	bind
38688	3	8926	7	NULL	NULL	0	NULL	apolipoprotein H	NULL		mediates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_neurobiolaging_20_4_457_s_139	10604441	A "`hitchhiker"` method of cell entry has been suggested also for hepatitis B virus (HBV) bound to HDL or chylomicrons (this binding being mediated by apolipoprotein H), with the HBV-LP complex binding to hepatocytes via the LDL receptor (LDLR) or the LDLR-related protein/ 2-macroglogulin receptor (LRP) [  60].	bind
38689	4	8926	7	NULL	NULL	0	NULL	apolipoprotein H	NULL		mediates	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_neurobiolaging_20_4_457_s_139	10604441	A "`hitchhiker"` method of cell entry has been suggested also for hepatitis B virus (HBV) bound to HDL or chylomicrons (this binding being mediated by apolipoprotein H), with the HBV-LP complex binding to hepatocytes via the LDL receptor (LDLR) or the LDLR-related protein/ 2-macroglogulin receptor (LRP) [  60].	bind
38690	5	8926	7	NULL	NULL	0	NULL	HBV-LP complex 	NULL		bind	NULL				hepatocytes	NULL				NULL		0	NULL	NULL	NULL	gw60_neurobiolaging_20_4_457_s_139	10604441	A "`hitchhiker"` method of cell entry has been suggested also for hepatitis B virus (HBV) bound to HDL or chylomicrons (this binding being mediated by apolipoprotein H), with the HBV-LP complex binding to hepatocytes via the LDL receptor (LDLR) or the LDLR-related protein/ 2-macroglogulin receptor (LRP) [  60].	bind
38691	6	8926	7	NULL	NULL	0	NULL	statement 5	NULL		via	NULL				LDLR	NULL				NULL		0	NULL	NULL	NULL	gw60_neurobiolaging_20_4_457_s_139	10604441	A "`hitchhiker"` method of cell entry has been suggested also for hepatitis B virus (HBV) bound to HDL or chylomicrons (this binding being mediated by apolipoprotein H), with the HBV-LP complex binding to hepatocytes via the LDL receptor (LDLR) or the LDLR-related protein/ 2-macroglogulin receptor (LRP) [  60].	bind
38692	7	8926	7	NULL	NULL	0	NULL	statement 5	NULL		via	NULL				LRP	NULL				NULL		0	NULL	NULL	NULL	gw60_neurobiolaging_20_4_457_s_139	10604441	A "`hitchhiker"` method of cell entry has been suggested also for hepatitis B virus (HBV) bound to HDL or chylomicrons (this binding being mediated by apolipoprotein H), with the HBV-LP complex binding to hepatocytes via the LDL receptor (LDLR) or the LDLR-related protein/ 2-macroglogulin receptor (LRP) [  60].	bind
38693	8	8926	7	NULL	NULL	0	NULL	HBV	NULL		is	NULL				hepatitis B virus	NULL				NULL		0	NULL	NULL	NULL	gw60_neurobiolaging_20_4_457_s_139	10604441	A "`hitchhiker"` method of cell entry has been suggested also for hepatitis B virus (HBV) bound to HDL or chylomicrons (this binding being mediated by apolipoprotein H), with the HBV-LP complex binding to hepatocytes via the LDL receptor (LDLR) or the LDLR-related protein/ 2-macroglogulin receptor (LRP) [  60].	bind
38694	9	8926	7	NULL	NULL	0	NULL	LDLR	NULL		is	NULL				LDL receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_neurobiolaging_20_4_457_s_139	10604441	A "`hitchhiker"` method of cell entry has been suggested also for hepatitis B virus (HBV) bound to HDL or chylomicrons (this binding being mediated by apolipoprotein H), with the HBV-LP complex binding to hepatocytes via the LDL receptor (LDLR) or the LDLR-related protein/ 2-macroglogulin receptor (LRP) [  60].	bind
38695	10	8926	7	NULL	NULL	0	NULL	LRP	NULL		is	NULL				LDLR-related protein	NULL				NULL		0	NULL	NULL	NULL	gw60_neurobiolaging_20_4_457_s_139	10604441	A "`hitchhiker"` method of cell entry has been suggested also for hepatitis B virus (HBV) bound to HDL or chylomicrons (this binding being mediated by apolipoprotein H), with the HBV-LP complex binding to hepatocytes via the LDL receptor (LDLR) or the LDLR-related protein/ 2-macroglogulin receptor (LRP) [  60].	bind
38696	11	8926	7	10	NULL	0	NULL	2-macroglogulin receptor	NULL		is a synonym of	NULL				LRP 	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neurobiolaging_20_4_457_s_139	10604441	A "`hitchhiker"` method of cell entry has been suggested also for hepatitis B virus (HBV) bound to HDL or chylomicrons (this binding being mediated by apolipoprotein H), with the HBV-LP complex binding to hepatocytes via the LDL receptor (LDLR) or the LDLR-related protein/ 2-macroglogulin receptor (LRP) [  60].	bind
38697	12	8926	7	NULL	NULL	0	NULL	statement 6	NULL		is an alternative to	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw60_neurobiolaging_20_4_457_s_139	10604441	A "`hitchhiker"` method of cell entry has been suggested also for hepatitis B virus (HBV) bound to HDL or chylomicrons (this binding being mediated by apolipoprotein H), with the HBV-LP complex binding to hepatocytes via the LDL receptor (LDLR) or the LDLR-related protein/ 2-macroglogulin receptor (LRP) [  60].	bind
47033	13	8926	7	10	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_neurobiolaging_20_4_457_s_139	10604441	A "`hitchhiker"` method of cell entry has been suggested also for hepatitis B virus (HBV) bound to HDL or chylomicrons (this binding being mediated by apolipoprotein H), with the HBV-LP complex binding to hepatocytes via the LDL receptor (LDLR) or the LDLR-related protein/ 2-macroglogulin receptor (LRP) [  60].	bind
29794	1	8928	6	13	NULL	NULL	NULL	glycogen synthase	GP		bind		may			PP1C	GP				NULL	lysates of COS7 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_34_26074_s_81	10856301	A "`pull-down"` assay was used to test for binding of glycogen synthase and PP1C from lysates of COS7 cells.	bind
38698	1	8928	7	10	NULL	0	NULL	glycogen synthase	NULL		bind	NULL	may			PP1C	NULL				NULL	lysates of COS7 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_34_26074_s_81	10856301	A "`pull-down"` assay was used to test for binding of glycogen synthase and PP1C from lysates of COS7 cells.	bind
29795	1	8929	6	13	NULL	NULL	NULL	CNA	GP	Staphylococcus aureus	bind					collagen	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0560-0569_embo-j_24_24_16362049_s_1	16362049	A 'Collagen Hug' model for Staphylococcus aureus CNA binding to collagen..	bind
38699	1	8929	7	NULL	NULL	0	NULL	CNA	NULL	Staphylococcus aureus	bind	NULL				collagen	NULL				NULL		0	NULL	NULL	NULL	abs-batch0560-0569_embo-j_24_24_16362049_s_1	16362049	A 'Collagen Hug' model for Staphylococcus aureus CNA binding to collagen..	bind
29796	1	8931	6	13	NULL	NULL	NULL	CIS family protein	GP		bind					EPOR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29338_s_282	10882725	A , binding of the CIS family proteins with the EPOR.	bind
38703	1	8931	7	NULL	NULL	0	NULL	 CIS family protein	NULL		bind	NULL				EPOR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29338_s_282	10882725	A , binding of the CIS family proteins with the EPOR.	bind
29797	1	8932	6	13	NULL	NULL	NULL	cyclophilin A	GP	triple mutant	bind			ATM		cyclosporin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_13_761_s_57	9651680	A , the ATM triple mutant of cyclophilin A that binds cyclosporin and some cyclosporin derivatives  [70]  ;	bind
29798	2	8932	6	13	NULL	NULL	NULL	cyclophilin A	GP	triple mutant	bind			ATM		cyclosporin derivatives	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_13_761_s_57	9651680	A , the ATM triple mutant of cyclophilin A that binds cyclosporin and some cyclosporin derivatives  [70]  ;	bind
38704	1	8932	7	10	NULL	0	NULL	cyclophilin A	NULL	triple mutant	bind	NULL		ATM		cyclosporin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_13_761_s_57	9651680	A , the ATM triple mutant of cyclophilin A that binds cyclosporin and some cyclosporin derivatives  [70]  ;	bind
38705	2	8932	7	10	NULL	0	NULL	cyclophilin A	NULL	triple mutant	bind	NULL		ATM		 cyclosporin derivative	NULL				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_13_761_s_57	9651680	A , the ATM triple mutant of cyclophilin A that binds cyclosporin and some cyclosporin derivatives  [70]  ;	bind
29799	1	8935	6	13	NULL	NULL	NULL	FXR/RXR protein	GP		bind					BACS gene	GP	radiolabeled		IR-1 sequences	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_30_27703_s_138	12754200	A -  C, FXR/RXR proteins bind to radiolabeled IR-1  sequences from the BACS and BAT genes  with similar affinities as binding to an  IR-1 from the mouse IBABP gene.	bind
29800	2	8935	6	13	NULL	NULL	NULL	FXR/RXR protein	GP		bind					BAT gene	GP	radiolabeled		IR-1 sequences	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_30_27703_s_138	12754200	A -  C, FXR/RXR proteins bind to radiolabeled IR-1  sequences from the BACS and BAT genes  with similar affinities as binding to an  IR-1 from the mouse IBABP gene.	bind
29801	3	8935	6	13	NULL	NULL	NULL	FXR/RXR protein	GP		bind					IBABP gene	GP	mouse		IR-1 sequences	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_30_27703_s_138	12754200	A -  C, FXR/RXR proteins bind to radiolabeled IR-1  sequences from the BACS and BAT genes  with similar affinities as binding to an  IR-1 from the mouse IBABP gene.	bind
29802	4	8935	6	13	NULL	NULL	NULL	statement 1	Process	affinity of	is similar to					statement 3	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_30_27703_s_138	12754200	A -  C, FXR/RXR proteins bind to radiolabeled IR-1  sequences from the BACS and BAT genes  with similar affinities as binding to an  IR-1 from the mouse IBABP gene.	bind
29803	5	8935	6	13	NULL	NULL	NULL	statement 2	Process	affinity of	is similar to					statement 3	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_30_27703_s_138	12754200	A -  C, FXR/RXR proteins bind to radiolabeled IR-1  sequences from the BACS and BAT genes  with similar affinities as binding to an  IR-1 from the mouse IBABP gene.	bind
38706	1	8935	7	NULL	NULL	0	NULL	FXR/RXR proteins	NULL		bind	NULL				BACS gene	NULL	radiolabeled		IR-1 sequence	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_30_27703_s_138	12754200	A -  C, FXR/RXR proteins bind to radiolabeled IR-1  sequences from the BACS and BAT genes  with similar affinities as binding to an  IR-1 from the mouse IBABP gene.	bind
38707	2	8935	7	NULL	NULL	0	NULL	FXR/RXR proteins	NULL		bind	NULL				BAT genes	NULL	radiolabeled		IR-1 sequence	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_30_27703_s_138	12754200	A -  C, FXR/RXR proteins bind to radiolabeled IR-1  sequences from the BACS and BAT genes  with similar affinities as binding to an  IR-1 from the mouse IBABP gene.	bind
38708	3	8935	7	NULL	NULL	0	NULL	FXR/RXR proteins	NULL		bind	NULL				IBABP gene	NULL	mouse		IR-1 sequence	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_30_27703_s_138	12754200	A -  C, FXR/RXR proteins bind to radiolabeled IR-1  sequences from the BACS and BAT genes  with similar affinities as binding to an  IR-1 from the mouse IBABP gene.	bind
38709	4	8935	7	NULL	NULL	0	NULL	statement 1	NULL	affinity of	is similar to	NULL				statement 3	NULL	affinity of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_30_27703_s_138	12754200	A -  C, FXR/RXR proteins bind to radiolabeled IR-1  sequences from the BACS and BAT genes  with similar affinities as binding to an  IR-1 from the mouse IBABP gene.	bind
38710	5	8935	7	NULL	NULL	0	NULL	statement 2	NULL	affinity of	is similar to	NULL				statement 3	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_30_27703_s_138	12754200	A -  C, FXR/RXR proteins bind to radiolabeled IR-1  sequences from the BACS and BAT genes  with similar affinities as binding to an  IR-1 from the mouse IBABP gene.	bind
29806	2	8937	6	13	NULL	NULL	NULL	LPC	GP		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_1_13_s_71	9445250	A 0.5-mL portion of this solution was put on a NAP 5 column (Pharmacia) and eluted in water to separate [14]LPC bound to apoA-I - containing phospholipid particles from free [14]LPC.	bind
47077	1	8937	6	13	NULL	NULL	NULL	apoA-I	GP		contains					phospholipid particles	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_1_13_s_71	9445250	A 0.5-mL portion of this solution was put on a NAP 5 column (Pharmacia) and eluted in water to separate [14]LPC bound to apoA-I - containing phospholipid particles from free [14]LPC.	bind
38728	2	8937	7	10	NULL	0	NULL	LPC 			bind					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_1_13_s_71	9445250	A 0.5-mL portion of this solution was put on a NAP 5 column (Pharmacia) and eluted in water to separate [14]LPC bound to apoA-I - containing phospholipid particles from free [14]LPC.	bind
38729	1	8937	7	NULL	NULL	0	NULL	apoA-I	NULL		contain	NULL				phospholipid particles	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_18_1_13_s_71	9445250	A 0.5-mL portion of this solution was put on a NAP 5 column (Pharmacia) and eluted in water to separate [14]LPC bound to apoA-I - containing phospholipid particles from free [14]LPC.	bind
29807	1	8938	6	13	NULL	NULL	NULL	RII	GP		bind					ERM protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_1_35_s_57	9009265	A 1 muM concentration of the HT-31 peptide inhibited binding of [32]RII to all three ERM proteins (Figure  2).	bind
29808	2	8938	6	13	NULL	NULL	NULL	HT-31 peptide 	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_1_35_s_57	9009265	A 1 muM concentration of the HT-31 peptide inhibited binding of [32]RII to all three ERM proteins (Figure  2).	bind
38730	1	8938	7	10	NULL	0	NULL	RII			bind					ERM proteins					NULL		NULL	NULL	NULL	NULL	gw60_embo_16_1_35_s_57	9009265	A 1 muM concentration of the HT-31 peptide inhibited binding of [32]RII to all three ERM proteins (Figure  2).	bind
38731	2	8938	7	NULL	NULL	0	NULL	HT-31 peptide	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_16_1_35_s_57	9009265	A 1 muM concentration of the HT-31 peptide inhibited binding of [32]RII to all three ERM proteins (Figure  2).	bind
29849	1	8939	6	13	NULL	NULL	NULL	blr1 gene	GP		confers				360-bp 5'' flanking region	RA 	Chemical	response to			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_6_2423_s_266	14993281	A 1,360-bp 5''-flanking region of the  blr1 gene confers RA response and contains a distal 205-bp sequence necessary for response  A 5''-flanking region extending from -1096 to the 5' end of the first exon at +266 of the  blr1 gene confers response to RA.	bind
38732	1	8939	7	13	NULL	NULL	NULL	blr1 gene 	GP		confers				360-bp 5''-flanking region of	RA	Chemical	response to			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_6_2423_s_266	14993281	A 1,360-bp 5''-flanking region of the  blr1 gene confers RA response and contains a distal 205-bp sequence necessary for response  A 5''-flanking region extending from -1096 to the 5' end of the first exon at +266 of the  blr1 gene confers response to RA.	bind
38778	2	8939	7	13	NULL	NULL	NULL	blr1 gene	GP	distal	is necessary for				205-bp sequence	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_6_2423_s_266	14993281	A 1,360-bp 5''-flanking region of the  blr1 gene confers RA response and contains a distal 205-bp sequence necessary for response  A 5''-flanking region extending from -1096 to the 5' end of the first exon at +266 of the  blr1 gene confers response to RA.	bind
38783	3	8939	7	13	NULL	NULL	NULL				extend from				5''-flanking region	blr1 gene	GP			-1096	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_6_2423_s_266	14993281	A 1,360-bp 5''-flanking region of the  blr1 gene confers RA response and contains a distal 205-bp sequence necessary for response  A 5''-flanking region extending from -1096 to the 5' end of the first exon at +266 of the  blr1 gene confers response to RA.	bind
38784	4	8939	7	13	NULL	NULL	NULL				extend to				5''-flanking region	blr1 gene	GP			5' end of the first exon at +266	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_6_2423_s_266	14993281	A 1,360-bp 5''-flanking region of the  blr1 gene confers RA response and contains a distal 205-bp sequence necessary for response  A 5''-flanking region extending from -1096 to the 5' end of the first exon at +266 of the  blr1 gene confers response to RA.	bind
38786	5	8939	7	13	NULL	NULL	NULL	statement 3	Process		is necessary for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_6_2423_s_266	14993281	A 1,360-bp 5''-flanking region of the  blr1 gene confers RA response and contains a distal 205-bp sequence necessary for response  A 5''-flanking region extending from -1096 to the 5' end of the first exon at +266 of the  blr1 gene confers response to RA.	bind
38788	6	8939	7	13	NULL	NULL	NULL	statement 4	Process		is necessary for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_6_2423_s_266	14993281	A 1,360-bp 5''-flanking region of the  blr1 gene confers RA response and contains a distal 205-bp sequence necessary for response  A 5''-flanking region extending from -1096 to the 5' end of the first exon at +266 of the  blr1 gene confers response to RA.	bind
29809	1	8942	6	13	NULL	NULL	NULL	GTP S	Chemical		bind					G protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_38_3_403_s_186	10219978	A 1-week treatment regimen with the LiCl-containing diet did not influence [35]GTP  S binding to the G   proteins.	bind
29810	2	8942	6	13	NULL	NULL	NULL	LiCl	Chemical		does not influence					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_38_3_403_s_186	10219978	A 1-week treatment regimen with the LiCl-containing diet did not influence [35]GTP  S binding to the G   proteins.	bind
38797	1	8942	7	10	NULL	0	NULL	GTP S			bind					G proteins					NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_38_3_403_s_186	10219978	A 1-week treatment regimen with the LiCl-containing diet did not influence [35]GTP  S binding to the G   proteins.	bind
38798	2	8942	7	10	NULL	0	NULL	LiCl	NULL		does not influence	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_38_3_403_s_186	10219978	A 1-week treatment regimen with the LiCl-containing diet did not influence [35]GTP  S binding to the G   proteins.	bind
29811	1	8948	6	13	NULL	NULL	NULL	GLUT1 cDNA probe	NucleicAcid	human	bind					GLUT1 DNA	NucleicAcid	genomic			NULL		NULL	NULL	NULL	NULL	gw70_amjpathol_163_5_1873_s_44	14578187	A 1.66-kb human GLUT1 cDNA probe that binds to genomic  GLUT1 DNA immediately 3' to the point of insertion of the targeting construct was used as an adjacent probe to confirm insertion of the targeting construct inside the endogenous  GLUT1 gene of ES cells after homologous recombination.	bind
38805	1	8948	7	10	NULL	0	NULL	GLUT1 cDNA probe	NULL	human	bind	NULL				GLUT1 DNA	NULL	genomic			NULL		NULL	NULL	NULL	NULL	gw70_amjpathol_163_5_1873_s_44	14578187	A 1.66-kb human GLUT1 cDNA probe that binds to genomic  GLUT1 DNA immediately 3' to the point of insertion of the targeting construct was used as an adjacent probe to confirm insertion of the targeting construct inside the endogenous  GLUT1 gene of ES cells after homologous recombination.	bind
29812	1	8949	6	13	NULL	NULL	NULL	scFv2A-AP/S	GP	exogenous	bind					MBP-NIb	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_301_1_167_s_160	12535657	A 1/8  dilution of the agroinfiltrated plant extract inhibited binding of exogenous scFv2A-AP/S  to MBP-NIb by up to 32% ( Fig. 6).	bind
29813	2	8949	6	13	NULL	NULL	NULL	plant extract	Cell	agroinfiltrated	inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_301_1_167_s_160	12535657	A 1/8  dilution of the agroinfiltrated plant extract inhibited binding of exogenous scFv2A-AP/S  to MBP-NIb by up to 32% ( Fig. 6).	bind
38810	1	8949	7	10	NULL	0	NULL	scFv2A-AP/S	NULL	exogenous	bind	NULL				MBP-NIb	NULL				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_301_1_167_s_160	12535657	A 1/8  dilution of the agroinfiltrated plant extract inhibited binding of exogenous scFv2A-AP/S  to MBP-NIb by up to 32% ( Fig. 6).	bind
38811	2	8949	7	10	NULL	0	NULL	plant extract		agroinfiltrated	inhibits					statement 1					NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_301_1_167_s_160	12535657	A 1/8  dilution of the agroinfiltrated plant extract inhibited binding of exogenous scFv2A-AP/S  to MBP-NIb by up to 32% ( Fig. 6).	bind
29814	1	8951	6	13	NULL	NULL	NULL	EBNA2	GP		bind					CBF1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_13_4625_s_28	15070768	A 10-aa peptide was identified that was an effective competitor for EBNA2 binding to CBF1.	bind
38816	1	8951	7	NULL	NULL	0	NULL	EBNA2	NULL		bind	NULL				CBF1	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_101_13_4625_s_28	15070768	A 10-aa peptide was identified that was an effective competitor for EBNA2 binding to CBF1.	bind
29815	1	8952	6	13	NULL	NULL	NULL	HOAP	GP		bind			carboxyl terminal domain		HP1a	GP		hinge domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_36_34491_s_156	12826664	A 10-fold  molar excess of the HP1a-specific peptide was able to compete with binding of  the HOAP carboxyl terminal domain to the HP1a hinge domain, whereas the HP1b  and HP1c peptides were unable to compete even at a 100-fold molar excess.	bind
29816	2	8952	6	13	NULL	NULL	NULL	HP1a-specific peptide	GP		bind					HP1a	GP		hinge domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_36_34491_s_156	12826664	A 10-fold  molar excess of the HP1a-specific peptide was able to compete with binding of  the HOAP carboxyl terminal domain to the HP1a hinge domain, whereas the HP1b  and HP1c peptides were unable to compete even at a 100-fold molar excess.	bind
29817	3	8952	6	13	NULL	NULL	NULL	statement 1	Process		competes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_36_34491_s_156	12826664	A 10-fold  molar excess of the HP1a-specific peptide was able to compete with binding of  the HOAP carboxyl terminal domain to the HP1a hinge domain, whereas the HP1b  and HP1c peptides were unable to compete even at a 100-fold molar excess.	bind
29818	4	8952	6	13	NULL	NULL	NULL	HP1b peptide	GP		does not bind					Hp1a	GP		hinge domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_36_34491_s_156	12826664	A 10-fold  molar excess of the HP1a-specific peptide was able to compete with binding of  the HOAP carboxyl terminal domain to the HP1a hinge domain, whereas the HP1b  and HP1c peptides were unable to compete even at a 100-fold molar excess.	bind
29819	5	8952	6	13	NULL	NULL	NULL	HP1c peptide	GP		does not bind					HP1a	GP		hinge domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_36_34491_s_156	12826664	A 10-fold  molar excess of the HP1a-specific peptide was able to compete with binding of  the HOAP carboxyl terminal domain to the HP1a hinge domain, whereas the HP1b  and HP1c peptides were unable to compete even at a 100-fold molar excess.	bind
38818	1	8952	7	NULL	NULL	0	NULL	HOAP	NULL		bind	NULL		carboxyl terminal domain		HP1a	NULL		hinge domain		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_36_34491_s_156	12826664	A 10-fold  molar excess of the HP1a-specific peptide was able to compete with binding of  the HOAP carboxyl terminal domain to the HP1a hinge domain, whereas the HP1b  and HP1c peptides were unable to compete even at a 100-fold molar excess.	bind
38819	2	8952	7	10	NULL	0	NULL	statement 5	NULL		competes with	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_36_34491_s_156	12826664	A 10-fold  molar excess of the HP1a-specific peptide was able to compete with binding of  the HOAP carboxyl terminal domain to the HP1a hinge domain, whereas the HP1b  and HP1c peptides were unable to compete even at a 100-fold molar excess.	bind
38820	3	8952	7	NULL	NULL	0	NULL	HP1b peptide	NULL		unable to compete with	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_36_34491_s_156	12826664	A 10-fold  molar excess of the HP1a-specific peptide was able to compete with binding of  the HOAP carboxyl terminal domain to the HP1a hinge domain, whereas the HP1b  and HP1c peptides were unable to compete even at a 100-fold molar excess.	bind
38821	4	8952	7	NULL	NULL	0	NULL	HP1c peptide	NULL		unable to compete with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_36_34491_s_156	12826664	A 10-fold  molar excess of the HP1a-specific peptide was able to compete with binding of  the HOAP carboxyl terminal domain to the HP1a hinge domain, whereas the HP1b  and HP1c peptides were unable to compete even at a 100-fold molar excess.	bind
47078	5	8952	7	10	NULL	0	NULL	\tHP1a-specific peptide	NULL		bind	NULL				HP1a	NULL		hinge domain		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_36_34491_s_156	12826664	A 10-fold  molar excess of the HP1a-specific peptide was able to compete with binding of  the HOAP carboxyl terminal domain to the HP1a hinge domain, whereas the HP1b  and HP1c peptides were unable to compete even at a 100-fold molar excess.	bind
29820	1	8953	6	13	NULL	NULL	NULL	apoE protein	GP	full length	lowers					3H-LDL	GP	bound			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13333_s_262	16540478	A 10-fold dose of full-length apoE protein only lowered 34% of the bound 3H-LDL, whereas the same dose of apoE-DMPC lowered 58-59% of the bound 3H-LDL. The LDL-R binding ability of apoE-DMPC was higher than that of LDL at the same dose (20-fold), although apoE with or without DMPC did not show isoform specificity.	bind
29821	2	8953	6	13	NULL	NULL	NULL	apoE-DMPC	GP		lowers					3H-LDL	GP	bound			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13333_s_262	16540478	A 10-fold dose of full-length apoE protein only lowered 34% of the bound 3H-LDL, whereas the same dose of apoE-DMPC lowered 58-59% of the bound 3H-LDL. The LDL-R binding ability of apoE-DMPC was higher than that of LDL at the same dose (20-fold), although apoE with or without DMPC did not show isoform specificity.	bind
29822	3	8953	6	13	NULL	NULL	NULL	apoE-DMPC	GP		bind					LDL-R	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13333_s_262	16540478	A 10-fold dose of full-length apoE protein only lowered 34% of the bound 3H-LDL, whereas the same dose of apoE-DMPC lowered 58-59% of the bound 3H-LDL. The LDL-R binding ability of apoE-DMPC was higher than that of LDL at the same dose (20-fold), although apoE with or without DMPC did not show isoform specificity.	bind
29823	4	8953	6	13	NULL	NULL	NULL	LDL	GP		bind					apoE-DMPC	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13333_s_262	16540478	A 10-fold dose of full-length apoE protein only lowered 34% of the bound 3H-LDL, whereas the same dose of apoE-DMPC lowered 58-59% of the bound 3H-LDL. The LDL-R binding ability of apoE-DMPC was higher than that of LDL at the same dose (20-fold), although apoE with or without DMPC did not show isoform specificity.	bind
38822	1	8953	7	NULL	NULL	0	NULL	apoE protein	NULL	full-length	lowers	NULL				3H-LDL	NULL	bound			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13333_s_262	16540478	A 10-fold dose of full-length apoE protein only lowered 34% of the bound 3H-LDL, whereas the same dose of apoE-DMPC lowered 58-59% of the bound 3H-LDL. The LDL-R binding ability of apoE-DMPC was higher than that of LDL at the same dose (20-fold), although apoE with or without DMPC did not show isoform specificity.	bind
38823	2	8953	7	NULL	NULL	0	NULL	apoE-DMPC	NULL		lowers	NULL				 3H-LDL	NULL	bound			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13333_s_262	16540478	A 10-fold dose of full-length apoE protein only lowered 34% of the bound 3H-LDL, whereas the same dose of apoE-DMPC lowered 58-59% of the bound 3H-LDL. The LDL-R binding ability of apoE-DMPC was higher than that of LDL at the same dose (20-fold), although apoE with or without DMPC did not show isoform specificity.	bind
38824	3	8953	7	NULL	NULL	0	NULL	LDL-R	NULL		bind	NULL				apoE-DMPC	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_19_13333_s_262	16540478	A 10-fold dose of full-length apoE protein only lowered 34% of the bound 3H-LDL, whereas the same dose of apoE-DMPC lowered 58-59% of the bound 3H-LDL. The LDL-R binding ability of apoE-DMPC was higher than that of LDL at the same dose (20-fold), although apoE with or without DMPC did not show isoform specificity.	bind
38825	4	8953	7	NULL	NULL	0	NULL	LDL	NULL		bind	NULL				apoE-DMPC	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_19_13333_s_262	16540478	A 10-fold dose of full-length apoE protein only lowered 34% of the bound 3H-LDL, whereas the same dose of apoE-DMPC lowered 58-59% of the bound 3H-LDL. The LDL-R binding ability of apoE-DMPC was higher than that of LDL at the same dose (20-fold), although apoE with or without DMPC did not show isoform specificity.	bind
38826	5	8953	7	NULL	NULL	0	NULL	statement 3	NULL	binding of	is higher than	NULL				statement 4	NULL	binding of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_19_13333_s_262	16540478	A 10-fold dose of full-length apoE protein only lowered 34% of the bound 3H-LDL, whereas the same dose of apoE-DMPC lowered 58-59% of the bound 3H-LDL. The LDL-R binding ability of apoE-DMPC was higher than that of LDL at the same dose (20-fold), although apoE with or without DMPC did not show isoform specificity.	bind
29824	1	8954	6	13	NULL	NULL	NULL	GR	GP	phosphorylation of	is dependent on					Dex	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_29_26573_s_143	12000743	A 10-fold excess of ZK299 was not as effective at blocking the Dex-dependent phosphorylation of GR, presumably because of its lower affinity for the receptor.	bind
29825	2	8954	6	13	NULL	NULL	NULL	ZK299	Chemical		does not block		effectively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_29_26573_s_143	12000743	A 10-fold excess of ZK299 was not as effective at blocking the Dex-dependent phosphorylation of GR, presumably because of its lower affinity for the receptor.	bind
38827	1	8954	7	NULL	NULL	0	NULL	GR	NULL	 phosphorylation of	depends on	NULL				Dex	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26573_s_143	12000743	A 10-fold excess of ZK299 was not as effective at blocking the Dex-dependent phosphorylation of GR, presumably because of its lower affinity for the receptor.	bind
38828	2	8954	7	NULL	NULL	0	NULL	ZK299 	NULL		does not block	NULL	effectively			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26573_s_143	12000743	A 10-fold excess of ZK299 was not as effective at blocking the Dex-dependent phosphorylation of GR, presumably because of its lower affinity for the receptor.	bind
29826	1	8956	6	13	NULL	NULL	NULL	Tf-R	GP		bind		weakly			Tf	GP	bovine			NULL		NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_52_0_745_s_562	9891812	A 10-fold higher value was reported by Salmon et al ( 112), but this value is a priori implausible (as this high number of receptors could  occupy half the flagellar pocket wall), and it was based on inaccurate Tf binding  curves obtained with a Tf-R that binds bovine Tf weakly (cf  21,  125).	bind
38830	1	8956	7	NULL	NULL	0	NULL	 Tf-R	NULL		binds	NULL	weakly			Tf	NULL	bovine			NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_52_0_745_s_562	9891812	A 10-fold higher value was reported by Salmon et al ( 112), but this value is a priori implausible (as this high number of receptors could  occupy half the flagellar pocket wall), and it was based on inaccurate Tf binding  curves obtained with a Tf-R that binds bovine Tf weakly (cf  21,  125).	bind
29827	1	8957	6	13	NULL	NULL	NULL	MRP	GP		bind					PC/PS vesicles	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_34_19879_s_233	7650001	A 10-fold increase in Triton X-100,  e.g.  0.01%,  does not change the apparent partition coefficient for the binding of  MRP to PC/PS vesicles (4:1) (not shown).	bind
38831	1	8957	7	NULL	NULL	0	NULL	MRP	NULL		bind	NULL				PC/PS vesicles	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_34_19879_s_233	7650001	A 10-fold increase in Triton X-100,  e.g.  0.01%,  does not change the apparent partition coefficient for the binding of  MRP to PC/PS vesicles (4:1) (not shown).	bind
29828	1	8958	6	13	NULL	NULL	NULL	rpr	GP		bind				EcRE	EcR/USP heterodimer	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_3_445_s_186	10882130	A 10-fold molar excess of this mutated EcRE had no effect on formation of EcR/USP/ hsp27 EcRE complex, indicating that these conserved nucleotides are required for binding of the  rpr EcRE by the EcR/USP heterodimer (  Figure 6B, lane 9).	bind
29829	2	8958	6	13	NULL	NULL	NULL	statement 1	Process		forms a					EcR/USP/ hsp27 EcRE complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_3_445_s_186	10882130	A 10-fold molar excess of this mutated EcRE had no effect on formation of EcR/USP/ hsp27 EcRE complex, indicating that these conserved nucleotides are required for binding of the  rpr EcRE by the EcR/USP heterodimer (  Figure 6B, lane 9).	bind
29830	3	8958	6	13	NULL	NULL	NULL	EcRE	GP	mutant	has no effect on					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_3_445_s_186	10882130	A 10-fold molar excess of this mutated EcRE had no effect on formation of EcR/USP/ hsp27 EcRE complex, indicating that these conserved nucleotides are required for binding of the  rpr EcRE by the EcR/USP heterodimer (  Figure 6B, lane 9).	bind
38922	1	8958	7	10	NULL	0	NULL	EcR/USP heterodimer	NULL		bind	NULL				rpr	NULL			EcRE	NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_3_445_s_186	10882130	A 10-fold molar excess of this mutated EcRE had no effect on formation of EcR/USP/ hsp27 EcRE complex, indicating that these conserved nucleotides are required for binding of the  rpr EcRE by the EcR/USP heterodimer (  Figure 6B, lane 9).	bind
38923	2	8958	7	10	NULL	0	NULL	EcRE	NULL	mutant	does not affect	NULL				EcR/USP/ hsp27 EcRE complex	NULL	formation of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_3_445_s_186	10882130	A 10-fold molar excess of this mutated EcRE had no effect on formation of EcR/USP/ hsp27 EcRE complex, indicating that these conserved nucleotides are required for binding of the  rpr EcRE by the EcR/USP heterodimer (  Figure 6B, lane 9).	bind
38924	3	8958	7	NULL	NULL	0	NULL		NULL		is required for	NULL			conserved nucleotides	statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_5_3_445_s_186	10882130	A 10-fold molar excess of this mutated EcRE had no effect on formation of EcR/USP/ hsp27 EcRE complex, indicating that these conserved nucleotides are required for binding of the  rpr EcRE by the EcR/USP heterodimer (  Figure 6B, lane 9).	bind
29831	1	8960	6	13	NULL	NULL	NULL	AO	Chemical		bind					chromatin	Chromosome	sperm cell			NULL		NULL	NULL	NULL	NULL	abs-batch0760-0779_biull-eksp-biol-med_95_4_6831026_s_6	6831026	A 10-time decrease in the fluorescence of AO bound with sperm  cell chromatin as compared to F530 AO bound with lymphocyte chromatin  structure of the same individual supports the data on the over condensation  of sperm cell nuclear chromatin as compared to that in lymphocytes.	bind
29832	2	8960	6	13	NULL	NULL	NULL	AO	Chemical		bind					lymphocyte chromatin structure	Chromosome				NULL		NULL	NULL	NULL	NULL	abs-batch0760-0779_biull-eksp-biol-med_95_4_6831026_s_6	6831026	A 10-time decrease in the fluorescence of AO bound with sperm  cell chromatin as compared to F530 AO bound with lymphocyte chromatin  structure of the same individual supports the data on the over condensation  of sperm cell nuclear chromatin as compared to that in lymphocytes.	bind
38925	1	8960	7	10	NULL	0	NULL	chromatin 		sperm cell	bind					AO					NULL		NULL	NULL	NULL	NULL	abs-batch0760-0779_biull-eksp-biol-med_95_4_6831026_s_6	6831026	A 10-time decrease in the fluorescence of AO bound with sperm  cell chromatin as compared to F530 AO bound with lymphocyte chromatin  structure of the same individual supports the data on the over condensation  of sperm cell nuclear chromatin as compared to that in lymphocytes.	bind
38926	2	8960	7	NULL	NULL	0	NULL	lymphocyte chromatin structure	NULL		bind	NULL				AO	NULL			F530	NULL		0	NULL	NULL	NULL	abs-batch0760-0779_biull-eksp-biol-med_95_4_6831026_s_6	6831026	A 10-time decrease in the fluorescence of AO bound with sperm  cell chromatin as compared to F530 AO bound with lymphocyte chromatin  structure of the same individual supports the data on the over condensation  of sperm cell nuclear chromatin as compared to that in lymphocytes.	bind
29850	1	8963	6	13	NULL	NULL	NULL	LHR A	GP		bind					C4b	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_44_31160_s_112	10531307	A 100% value was assigned to the fraction of LHR A that bound to C4b- or iC3-Sepharose.	bind
29851	2	8963	6	13	NULL	NULL	NULL	LHR A	GP		bind					iC3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_44_31160_s_112	10531307	A 100% value was assigned to the fraction of LHR A that bound to C4b- or iC3-Sepharose.	bind
39339	1	8963	7	10	NULL	0	NULL	LHR A	NULL		bind	NULL				C4b	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_44_31160_s_112	10531307	A 100% value was assigned to the fraction of LHR A that bound to C4b- or iC3-Sepharose.	bind
39340	2	8963	7	10	NULL	0	NULL	LHR A	NULL		bind	NULL				iC3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_44_31160_s_112	10531307	A 100% value was assigned to the fraction of LHR A that bound to C4b- or iC3-Sepharose.	bind
29852	1	8964	6	13	NULL	NULL	NULL	oriR replication origin	NucleicAcid		bind				100 bp region	RepA protein plasmid	GP				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_62_2_434_s_337	9618448	A 100-bp region in the  oriR replication origin is continuously bound by the plasmid RepA protein to form the initiation complex.	bind
29853	2	8964	6	13	NULL	NULL	NULL	statement 1	Process		forms					initiation complex	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_62_2_434_s_337	9618448	A 100-bp region in the  oriR replication origin is continuously bound by the plasmid RepA protein to form the initiation complex.	bind
39341	1	8964	7	NULL	NULL	0	NULL	oriR replication origin	NULL		bind	NULL				plasmid RepA protein	NULL				NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_62_2_434_s_337	9618448	A 100-bp region in the  oriR replication origin is continuously bound by the plasmid RepA protein to form the initiation complex.	bind
39342	2	8964	7	NULL	NULL	0	NULL	statement 1	NULL		form	NULL				initiation complex	NULL				NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_62_2_434_s_337	9618448	A 100-bp region in the  oriR replication origin is continuously bound by the plasmid RepA protein to form the initiation complex.	bind
31152	1	8967	6	13	NULL	NULL	NULL	TEC1	GP		competes with				FRE	Ty1	GP			FRE	NULL		NULL	NULL	NULL	NULL	gw60_science_275_5304_1314_s_99	9036858	A 100-fold excess of the unlabeled  TEC1 FRE also eliminated binding to the  Ty1 FRE (Fig.  4A, lane 9), whereas  TEC1 FREs containing point mutations in either the PRE or TCS did not compete.	bind
31154	2	8967	6	13	NULL	NULL	NULL	TEC1 	GP	mutant	does not compete				FRE	Ty1	GP			FRE	NULL		NULL	NULL	NULL	NULL	gw60_science_275_5304_1314_s_99	9036858	A 100-fold excess of the unlabeled  TEC1 FRE also eliminated binding to the  Ty1 FRE (Fig.  4A, lane 9), whereas  TEC1 FREs containing point mutations in either the PRE or TCS did not compete.	bind
39345	1	8967	7	NULL	NULL	0	NULL	TEC1	NULL	unlabeled 	bind	NULL			FRE	Ty1	NULL			FRE	NULL		0	NULL	NULL	NULL	gw60_science_275_5304_1314_s_99	9036858	A 100-fold excess of the unlabeled  TEC1 FRE also eliminated binding to the  Ty1 FRE (Fig.  4A, lane 9), whereas  TEC1 FREs containing point mutations in either the PRE or TCS did not compete.	bind
39346	2	8967	7	NULL	NULL	0	NULL	TEC1	NULL	point mutant	does not compete with	NULL			FREs containing PRE	statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_science_275_5304_1314_s_99	9036858	A 100-fold excess of the unlabeled  TEC1 FRE also eliminated binding to the  Ty1 FRE (Fig.  4A, lane 9), whereas  TEC1 FREs containing point mutations in either the PRE or TCS did not compete.	bind
39347	3	8967	7	NULL	NULL	0	NULL	TEC1	NULL	point mutant	does not compete with	NULL			FREs containing TCS	statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_science_275_5304_1314_s_99	9036858	A 100-fold excess of the unlabeled  TEC1 FRE also eliminated binding to the  Ty1 FRE (Fig.  4A, lane 9), whereas  TEC1 FREs containing point mutations in either the PRE or TCS did not compete.	bind
39348	4	8967	7	10	NULL	0	NULL	TEC1	NULL	excess of;;unlabeled	eliminate	NULL			FRE	statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_science_275_5304_1314_s_99	9036858	A 100-fold excess of the unlabeled  TEC1 FRE also eliminated binding to the  Ty1 FRE (Fig.  4A, lane 9), whereas  TEC1 FREs containing point mutations in either the PRE or TCS did not compete.	bind
30321	1	8968	6	13	NULL	NULL	NULL	Pab1p	GP		bind					MFA2	NucleicAcid	capped		3'' UTR	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9753_s_109	16260593	A 100-fold excess of unlabeled uncapped MFA2 or excess unlabeled capped pGEM4 polylinker (Cap A0) or 100 ng of poly(C) failed to compete Pab1p bound to capped MFA2 3''-UTR (Fig.  2A, lanes 3 to 6 compared to lanes 2 and 6).	bind
30322	2	8968	6	13	NULL	NULL	NULL	MFA2	NucleicAcid	unlabeled;;uncapped	failed to compete					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9753_s_109	16260593	A 100-fold excess of unlabeled uncapped MFA2 or excess unlabeled capped pGEM4 polylinker (Cap A0) or 100 ng of poly(C) failed to compete Pab1p bound to capped MFA2 3''-UTR (Fig.  2A, lanes 3 to 6 compared to lanes 2 and 6).	bind
30323	3	8968	6	13	NULL	NULL	NULL	MFA2	NucleicAcid	unlabeled;;uncapped	failed to compete					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9753_s_109	16260593	A 100-fold excess of unlabeled uncapped MFA2 or excess unlabeled capped pGEM4 polylinker (Cap A0) or 100 ng of poly(C) failed to compete Pab1p bound to capped MFA2 3''-UTR (Fig.  2A, lanes 3 to 6 compared to lanes 2 and 6).	bind
56167	4	8968	6	13	NULL	NULL	NULL	poly(C)	Chemical		failed to compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9753_s_109	16260593	A 100-fold excess of unlabeled uncapped MFA2 or excess unlabeled capped pGEM4 polylinker (Cap A0) or 100 ng of poly(C) failed to compete Pab1p bound to capped MFA2 3''-UTR (Fig.  2A, lanes 3 to 6 compared to lanes 2 and 6).	bind
39349	1	8968	7	10	NULL	0	NULL	Pab1p	NULL		bind	NULL				MFA2	NULL	capped	3''-UTR		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9753_s_109	16260593	A 100-fold excess of unlabeled uncapped MFA2 or excess unlabeled capped pGEM4 polylinker (Cap A0) or 100 ng of poly(C) failed to compete Pab1p bound to capped MFA2 3''-UTR (Fig.  2A, lanes 3 to 6 compared to lanes 2 and 6).	bind
39350	2	8968	7	10	NULL	0	NULL	MFA2		unlabeled;;uncapped	fail to compete with					statement 1					NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9753_s_109	16260593	A 100-fold excess of unlabeled uncapped MFA2 or excess unlabeled capped pGEM4 polylinker (Cap A0) or 100 ng of poly(C) failed to compete Pab1p bound to capped MFA2 3''-UTR (Fig.  2A, lanes 3 to 6 compared to lanes 2 and 6).	bind
39351	3	8968	7	10	NULL	0	NULL	pGEM4 polylinker		unlabeled;;uncapped	fail to compete with					statement 1					NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_22_9753_s_109	16260593	A 100-fold excess of unlabeled uncapped MFA2 or excess unlabeled capped pGEM4 polylinker (Cap A0) or 100 ng of poly(C) failed to compete Pab1p bound to capped MFA2 3''-UTR (Fig.  2A, lanes 3 to 6 compared to lanes 2 and 6).	bind
39372	4	8968	7	NULL	NULL	0	NULL	poly(C)	NULL		fail to compete with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_22_9753_s_109	16260593	A 100-fold excess of unlabeled uncapped MFA2 or excess unlabeled capped pGEM4 polylinker (Cap A0) or 100 ng of poly(C) failed to compete Pab1p bound to capped MFA2 3''-UTR (Fig.  2A, lanes 3 to 6 compared to lanes 2 and 6).	bind
30325	1	8969	6	13	NULL	NULL	NULL			radiolabelled;;Drosophila	bind				IRE	IRP1	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_febslett_436_3_476_s_167	9801172	A 100-fold molar excess of both cold human ferritin H like IRE (I-12.CAT, lane 4 in  Fig. 1B) and cold human ferritin H IRE (pSPT-fer, lane 5 in  Fig. 1B) significantly reduced the binding of the radiolabelled  Drosophila IRE to the human IRP1, whereas a 100-fold molar excess of the human mutated IRE was without any affect (lane 3 in  Fig. 1B).	bind
30326	2	8969	6	13	NULL	NULL	NULL	ferritin H like	GP	cold;;human	reduces		significantly		IRE	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_436_3_476_s_167	9801172	A 100-fold molar excess of both cold human ferritin H like IRE (I-12.CAT, lane 4 in  Fig. 1B) and cold human ferritin H IRE (pSPT-fer, lane 5 in  Fig. 1B) significantly reduced the binding of the radiolabelled  Drosophila IRE to the human IRP1, whereas a 100-fold molar excess of the human mutated IRE was without any affect (lane 3 in  Fig. 1B).	bind
30327	3	8969	6	13	NULL	NULL	NULL	ferritin H 	GP	cold;;human	reduces		significantly		IRE	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_436_3_476_s_167	9801172	A 100-fold molar excess of both cold human ferritin H like IRE (I-12.CAT, lane 4 in  Fig. 1B) and cold human ferritin H IRE (pSPT-fer, lane 5 in  Fig. 1B) significantly reduced the binding of the radiolabelled  Drosophila IRE to the human IRP1, whereas a 100-fold molar excess of the human mutated IRE was without any affect (lane 3 in  Fig. 1B).	bind
30328	4	8969	6	13	NULL	NULL	NULL	IRE	GP	human;;mutant	does not affect					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_436_3_476_s_167	9801172	A 100-fold molar excess of both cold human ferritin H like IRE (I-12.CAT, lane 4 in  Fig. 1B) and cold human ferritin H IRE (pSPT-fer, lane 5 in  Fig. 1B) significantly reduced the binding of the radiolabelled  Drosophila IRE to the human IRP1, whereas a 100-fold molar excess of the human mutated IRE was without any affect (lane 3 in  Fig. 1B).	bind
39373	1	8969	7	10	NULL	0	NULL		NULL	radiolabelled;;Drosophila	bind	NULL			IRE	IRP1	NULL	human			NULL		NULL	NULL	NULL	NULL	gw60_febslett_436_3_476_s_167	9801172	A 100-fold molar excess of both cold human ferritin H like IRE (I-12.CAT, lane 4 in  Fig. 1B) and cold human ferritin H IRE (pSPT-fer, lane 5 in  Fig. 1B) significantly reduced the binding of the radiolabelled  Drosophila IRE to the human IRP1, whereas a 100-fold molar excess of the human mutated IRE was without any affect (lane 3 in  Fig. 1B).	bind
39374	2	8969	7	10	NULL	0	NULL	ferritin H like	NULL	cold;;human	reduce	NULL	significantly		IRE	statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_febslett_436_3_476_s_167	9801172	A 100-fold molar excess of both cold human ferritin H like IRE (I-12.CAT, lane 4 in  Fig. 1B) and cold human ferritin H IRE (pSPT-fer, lane 5 in  Fig. 1B) significantly reduced the binding of the radiolabelled  Drosophila IRE to the human IRP1, whereas a 100-fold molar excess of the human mutated IRE was without any affect (lane 3 in  Fig. 1B).	bind
39375	3	8969	7	10	NULL	0	NULL	ferritin H	NULL	cold;;human	reduce	NULL	significantly		 IRE	statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_febslett_436_3_476_s_167	9801172	A 100-fold molar excess of both cold human ferritin H like IRE (I-12.CAT, lane 4 in  Fig. 1B) and cold human ferritin H IRE (pSPT-fer, lane 5 in  Fig. 1B) significantly reduced the binding of the radiolabelled  Drosophila IRE to the human IRP1, whereas a 100-fold molar excess of the human mutated IRE was without any affect (lane 3 in  Fig. 1B).	bind
39376	4	8969	7	10	NULL	0	NULL		NULL	human;;mutant	does not affect	NULL			IRE	statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_febslett_436_3_476_s_167	9801172	A 100-fold molar excess of both cold human ferritin H like IRE (I-12.CAT, lane 4 in  Fig. 1B) and cold human ferritin H IRE (pSPT-fer, lane 5 in  Fig. 1B) significantly reduced the binding of the radiolabelled  Drosophila IRE to the human IRP1, whereas a 100-fold molar excess of the human mutated IRE was without any affect (lane 3 in  Fig. 1B).	bind
30329	1	8970	6	13	NULL	NULL	NULL	KKLF	GP		does not bind									SpI site (GGCGGG)	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7319_s_120	10982849	A 100-fold molar excess of cold SpI oligonucleotide (lane 3) did not compete with the GA element, suggesting that KKLF could not bind to the SpI site (GGCGGG).	bind
30330	2	8970	6	13	NULL	NULL	NULL	SpI oligonucleotide	NucleicAcid	cold	does not compete with									GA element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7319_s_120	10982849	A 100-fold molar excess of cold SpI oligonucleotide (lane 3) did not compete with the GA element, suggesting that KKLF could not bind to the SpI site (GGCGGG).	bind
39377	1	8970	7	10	NULL	0	NULL	KKLF	NULL		does not bind	NULL					NULL			SpI site (GGCGGG)	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7319_s_120	10982849	A 100-fold molar excess of cold SpI oligonucleotide (lane 3) did not compete with the GA element, suggesting that KKLF could not bind to the SpI site (GGCGGG).	bind
39378	2	8970	7	10	NULL	0	NULL	SpI oligonucleotide	NULL	cold	does not compete with	NULL					NULL			GA element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7319_s_120	10982849	A 100-fold molar excess of cold SpI oligonucleotide (lane 3) did not compete with the GA element, suggesting that KKLF could not bind to the SpI site (GGCGGG).	bind
30331	1	8971	6	13	NULL	NULL	NULL	TFPI	GP		bind					VLDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_15_12241_s_209	11278667	A 100-fold molar excess of RAP blocked more than 95% of TFPI binding to VLDL receptor.	bind
30332	2	8971	6	13	NULL	NULL	NULL	RAP	GP	excess of	block					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_15_12241_s_209	11278667	A 100-fold molar excess of RAP blocked more than 95% of TFPI binding to VLDL receptor.	bind
39379	1	8971	7	NULL	NULL	0	NULL	TFPI	NULL		bind	NULL				VLDL receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_15_12241_s_209	11278667	A 100-fold molar excess of RAP blocked more than 95% of TFPI binding to VLDL receptor.	bind
39380	2	8971	7	10	NULL	0	NULL	RAP		excess	blocks					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_15_12241_s_209	11278667	A 100-fold molar excess of RAP blocked more than 95% of TFPI binding to VLDL receptor.	bind
30333	1	8972	6	13	NULL	NULL	NULL	TFPI	GP	125I	bind					TSP-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_31715_s_180	10922378	A 100-fold molar excess of TFPI-160 had no effect on the binding of 125I-TFPI to TSP-1, whereas a 100-fold molar excess of K1K2C decreased binding to 15% (Fig.  6 B), demonstrating that the C-terminal region of TFPI has a critical role in the binding of TFPI to TSP-1.	bind
30334	2	8972	6	13	NULL	NULL	NULL	K1K2C	GP	excess of	decreases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_31715_s_180	10922378	A 100-fold molar excess of TFPI-160 had no effect on the binding of 125I-TFPI to TSP-1, whereas a 100-fold molar excess of K1K2C decreased binding to 15% (Fig.  6 B), demonstrating that the C-terminal region of TFPI has a critical role in the binding of TFPI to TSP-1.	bind
30335	3	8972	6	13	NULL	NULL	NULL	TFPI	GP		plays a role in			C-terminal region		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_31715_s_180	10922378	A 100-fold molar excess of TFPI-160 had no effect on the binding of 125I-TFPI to TSP-1, whereas a 100-fold molar excess of K1K2C decreased binding to 15% (Fig.  6 B), demonstrating that the C-terminal region of TFPI has a critical role in the binding of TFPI to TSP-1.	bind
30336	4	8972	6	13	NULL	NULL	NULL	TFPI-160	GP	excess of	had no effect on					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_31715_s_180	10922378	A 100-fold molar excess of TFPI-160 had no effect on the binding of 125I-TFPI to TSP-1, whereas a 100-fold molar excess of K1K2C decreased binding to 15% (Fig.  6 B), demonstrating that the C-terminal region of TFPI has a critical role in the binding of TFPI to TSP-1.	bind
39381	1	8972	7	10	NULL	0	NULL	TFPI	NULL	125I	bind	NULL				TSP-1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_31715_s_180	10922378	A 100-fold molar excess of TFPI-160 had no effect on the binding of 125I-TFPI to TSP-1, whereas a 100-fold molar excess of K1K2C decreased binding to 15% (Fig.  6 B), demonstrating that the C-terminal region of TFPI has a critical role in the binding of TFPI to TSP-1.	bind
39382	2	8972	7	10	NULL	0	NULL	TFPI-160		excess	does not affect					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_31715_s_180	10922378	A 100-fold molar excess of TFPI-160 had no effect on the binding of 125I-TFPI to TSP-1, whereas a 100-fold molar excess of K1K2C decreased binding to 15% (Fig.  6 B), demonstrating that the C-terminal region of TFPI has a critical role in the binding of TFPI to TSP-1.	bind
39383	3	8972	7	10	NULL	0	NULL	K1K2C		excess	decrease					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_31715_s_180	10922378	A 100-fold molar excess of TFPI-160 had no effect on the binding of 125I-TFPI to TSP-1, whereas a 100-fold molar excess of K1K2C decreased binding to 15% (Fig.  6 B), demonstrating that the C-terminal region of TFPI has a critical role in the binding of TFPI to TSP-1.	bind
39384	4	8972	7	NULL	NULL	0	NULL	TFPI	NULL		is critical for	NULL		C-terminal region of		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_41_31715_s_180	10922378	A 100-fold molar excess of TFPI-160 had no effect on the binding of 125I-TFPI to TSP-1, whereas a 100-fold molar excess of K1K2C decreased binding to 15% (Fig.  6 B), demonstrating that the C-terminal region of TFPI has a critical role in the binding of TFPI to TSP-1.	bind
30337	1	8973	6	13	NULL	NULL	NULL	OBP	GP		is					octamer binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_21_7712_s_492	12370317	A 100-kD HeLa cell octamer binding protein (OBP 100) interacts differently with two separate octamer-related sequences within the SV40 enhancer.	bind
30338	2	8973	6	13	NULL	NULL	NULL	OBP 100	GP		interacts		differently			SV40	GP			octamer-related sequences of enhancer	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_21_7712_s_492	12370317	A 100-kD HeLa cell octamer binding protein (OBP 100) interacts differently with two separate octamer-related sequences within the SV40 enhancer.	bind
39385	1	8973	7	10	NULL	0	NULL	OBP 100			interacts with		differently			SV40				octamer-related sequences within enhancer	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_21_7712_s_492	12370317	A 100-kD HeLa cell octamer binding protein (OBP 100) interacts differently with two separate octamer-related sequences within the SV40 enhancer.	bind
39386	2	8973	7	NULL	NULL	0	NULL	OBP 100	NULL		is	NULL				100-kD HeLa cell octamer binding protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_21_7712_s_492	12370317	A 100-kD HeLa cell octamer binding protein (OBP 100) interacts differently with two separate octamer-related sequences within the SV40 enhancer.	bind
30340	1	8978	6	13	NULL	NULL	NULL	Kes1p	GP		defines			205-314		Kes1p	GP	putative	PH domain		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_1_63_s_106	11916983	A 110 amino acid region of Kes1p (residues 205 - 314) that defines the putative Kes1p PH domain ( Fig. 2 B) also binds IP3 photo-probe (unpublished data).	bind
30341	2	8978	6	13	NULL	NULL	NULL	statement 1	GP		bind					IP3 photo-probe	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_1_63_s_106	11916983	A 110 amino acid region of Kes1p (residues 205 - 314) that defines the putative Kes1p PH domain ( Fig. 2 B) also binds IP3 photo-probe (unpublished data).	bind
39396	1	8978	7	10	NULL	0	NULL	Kes1p			defines			110 amino acid region 205 - 314		Kes1p		putative	 PH domain		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_157_1_63_s_106	11916983	A 110 amino acid region of Kes1p (residues 205 - 314) that defines the putative Kes1p PH domain ( Fig. 2 B) also binds IP3 photo-probe (unpublished data).	bind
39398	2	8978	7	NULL	NULL	0	NULL	statement 1	NULL		binds	NULL				IP3 photo-probe 	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_157_1_63_s_106	11916983	A 110 amino acid region of Kes1p (residues 205 - 314) that defines the putative Kes1p PH domain ( Fig. 2 B) also binds IP3 photo-probe (unpublished data).	bind
30373	1	8979	6	13	NULL	NULL	NULL	Pce1	GP		is a type of					guanylyltransferase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_22_19639_s_8	11893740	A 116-amino acid fragment of the guanylyltransferase Pce1 suffices for binding to the Spt5 C-terminal domain (CTD) but not for binding to the Pol-II CTD. Pct1 and Pce1 can bind simultaneously to the Spt5 CTD  in vitro.	bind
30374	2	8979	6	13	NULL	NULL	NULL	CTD	GP		is					C-terminal domain	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_22_19639_s_8	11893740	A 116-amino acid fragment of the guanylyltransferase Pce1 suffices for binding to the Spt5 C-terminal domain (CTD) but not for binding to the Pol-II CTD. Pct1 and Pce1 can bind simultaneously to the Spt5 CTD  in vitro.	bind
30375	3	8979	6	13	NULL	NULL	NULL	Pct1	GP		bind					Spt5	GP		CTD		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_22_19639_s_8	11893740	A 116-amino acid fragment of the guanylyltransferase Pce1 suffices for binding to the Spt5 C-terminal domain (CTD) but not for binding to the Pol-II CTD. Pct1 and Pce1 can bind simultaneously to the Spt5 CTD  in vitro.	bind
30376	4	8979	6	13	NULL	NULL	NULL	Pce1	GP		bind					Spt5	GP		CTD		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_22_19639_s_8	11893740	A 116-amino acid fragment of the guanylyltransferase Pce1 suffices for binding to the Spt5 C-terminal domain (CTD) but not for binding to the Pol-II CTD. Pct1 and Pce1 can bind simultaneously to the Spt5 CTD  in vitro.	bind
30377	5	8979	6	13	NULL	NULL	NULL	statement 3	Process		occurs simultaneously with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_22_19639_s_8	11893740	A 116-amino acid fragment of the guanylyltransferase Pce1 suffices for binding to the Spt5 C-terminal domain (CTD) but not for binding to the Pol-II CTD. Pct1 and Pce1 can bind simultaneously to the Spt5 CTD  in vitro.	bind
31156	6	8979	6	13	NULL	NULL	NULL	Pce1	GP		bind			116-amino acid fragment		Spt5	GP		CTD		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_22_19639_s_8	11893740	A 116-amino acid fragment of the guanylyltransferase Pce1 suffices for binding to the Spt5 C-terminal domain (CTD) but not for binding to the Pol-II CTD. Pct1 and Pce1 can bind simultaneously to the Spt5 CTD  in vitro.	bind
31157	7	8979	6	13	NULL	NULL	NULL	Pce1	GP		does not bind			116-amino acid fragment		Pol-II	GP		CTD		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_22_19639_s_8	11893740	A 116-amino acid fragment of the guanylyltransferase Pce1 suffices for binding to the Spt5 C-terminal domain (CTD) but not for binding to the Pol-II CTD. Pct1 and Pce1 can bind simultaneously to the Spt5 CTD  in vitro.	bind
39411	1	8979	7	10	NULL	0	NULL	Pce1	NULL		bind	NULL		116-amino acid fragment of		Spt5 	NULL		CTD		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_22_19639_s_8	11893740	A 116-amino acid fragment of the guanylyltransferase Pce1 suffices for binding to the Spt5 C-terminal domain (CTD) but not for binding to the Pol-II CTD. Pct1 and Pce1 can bind simultaneously to the Spt5 CTD  in vitro.	bind
39413	2	8979	7	10	NULL	0	NULL	Pce1	NULL		does not bind	NULL		116-amino acid fragment of		Pol-II 	NULL		CTD		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_22_19639_s_8	11893740	A 116-amino acid fragment of the guanylyltransferase Pce1 suffices for binding to the Spt5 C-terminal domain (CTD) but not for binding to the Pol-II CTD. Pct1 and Pce1 can bind simultaneously to the Spt5 CTD  in vitro.	bind
39414	3	8979	7	NULL	NULL	0	NULL	Pct1	NULL		bind	NULL				Spt5 	NULL		CTD		NULL	in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_277_22_19639_s_8	11893740	A 116-amino acid fragment of the guanylyltransferase Pce1 suffices for binding to the Spt5 C-terminal domain (CTD) but not for binding to the Pol-II CTD. Pct1 and Pce1 can bind simultaneously to the Spt5 CTD  in vitro.	bind
39417	4	8979	7	NULL	NULL	0	NULL	Pce1 	NULL		bind	NULL				Spt5 	NULL		CTD		NULL	in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_277_22_19639_s_8	11893740	A 116-amino acid fragment of the guanylyltransferase Pce1 suffices for binding to the Spt5 C-terminal domain (CTD) but not for binding to the Pol-II CTD. Pct1 and Pce1 can bind simultaneously to the Spt5 CTD  in vitro.	bind
39420	5	8979	7	NULL	NULL	0	NULL	statement 3	NULL		occur simultaneously with	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_22_19639_s_8	11893740	A 116-amino acid fragment of the guanylyltransferase Pce1 suffices for binding to the Spt5 C-terminal domain (CTD) but not for binding to the Pol-II CTD. Pct1 and Pce1 can bind simultaneously to the Spt5 CTD  in vitro.	bind
39421	6	8979	7	NULL	NULL	0	NULL	CTD	NULL		is	NULL					NULL		C-terminal domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_22_19639_s_8	11893740	A 116-amino acid fragment of the guanylyltransferase Pce1 suffices for binding to the Spt5 C-terminal domain (CTD) but not for binding to the Pol-II CTD. Pct1 and Pce1 can bind simultaneously to the Spt5 CTD  in vitro.	bind
47080	7	8979	7	10	NULL	0	NULL	Pce1	NULL		is a type of	NULL				guanylyltransferase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_22_19639_s_8	11893740	A 116-amino acid fragment of the guanylyltransferase Pce1 suffices for binding to the Spt5 C-terminal domain (CTD) but not for binding to the Pol-II CTD. Pct1 and Pce1 can bind simultaneously to the Spt5 CTD  in vitro.	bind
30378	1	8980	6	13	NULL	NULL	NULL	VEGF	GP	radiolabeled	bind					KDR receptor	GP				NULL	HUVEC	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_4_793_s_70	12646239	A 12 amino acid peptide corresponding to residueS 125-136 of the VEGF189 sequence is an effective inhibitor of radiolabelled VEGF binding to KDR and neuropilin-1  receptors in HUVECs and VEGF-dependent angiogenesis in an in vitro assay [ 22].	bind
30379	2	8980	6	13	NULL	NULL	NULL	VEGF	GP	radiolabeled	bind					neuropilin-1 receptor	GP				NULL	HUVEC	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_4_793_s_70	12646239	A 12 amino acid peptide corresponding to residueS 125-136 of the VEGF189 sequence is an effective inhibitor of radiolabelled VEGF binding to KDR and neuropilin-1  receptors in HUVECs and VEGF-dependent angiogenesis in an in vitro assay [ 22].	bind
30380	3	8980	6	13	NULL	NULL	NULL	VEGF189 peptide	GP		inhibits		effectively	residues 125-136		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_4_793_s_70	12646239	A 12 amino acid peptide corresponding to residueS 125-136 of the VEGF189 sequence is an effective inhibitor of radiolabelled VEGF binding to KDR and neuropilin-1  receptors in HUVECs and VEGF-dependent angiogenesis in an in vitro assay [ 22].	bind
30381	4	8980	6	13	NULL	NULL	NULL	VEGF189 peptide	GP		inhibits		effectively	residues 125-136		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_4_793_s_70	12646239	A 12 amino acid peptide corresponding to residueS 125-136 of the VEGF189 sequence is an effective inhibitor of radiolabelled VEGF binding to KDR and neuropilin-1  receptors in HUVECs and VEGF-dependent angiogenesis in an in vitro assay [ 22].	bind
30382	5	8980	6	13	NULL	NULL	NULL	angiogenesis	Process		is dependent on					VEGF	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_4_793_s_70	12646239	A 12 amino acid peptide corresponding to residueS 125-136 of the VEGF189 sequence is an effective inhibitor of radiolabelled VEGF binding to KDR and neuropilin-1  receptors in HUVECs and VEGF-dependent angiogenesis in an in vitro assay [ 22].	bind
30383	6	8980	6	13	NULL	NULL	NULL	VEGF189 peptide	GP		inhibits		effectively	residues 125-136		statement 5	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_4_793_s_70	12646239	A 12 amino acid peptide corresponding to residueS 125-136 of the VEGF189 sequence is an effective inhibitor of radiolabelled VEGF binding to KDR and neuropilin-1  receptors in HUVECs and VEGF-dependent angiogenesis in an in vitro assay [ 22].	bind
39425	1	8980	7	NULL	NULL	0	NULL	VEGF	NULL	radiolabelled 	bind	NULL				KDR	NULL				NULL	HUVECs	0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_4_793_s_70	12646239	A 12 amino acid peptide corresponding to residueS 125-136 of the VEGF189 sequence is an effective inhibitor of radiolabelled VEGF binding to KDR and neuropilin-1  receptors in HUVECs and VEGF-dependent angiogenesis in an in vitro assay [ 22].	bind
39427	2	8980	7	NULL	NULL	0	NULL	VEGF	NULL	radiolabelled	bind	NULL				neuropilin-1 receptors	NULL				NULL	HUVECs	0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_4_793_s_70	12646239	A 12 amino acid peptide corresponding to residueS 125-136 of the VEGF189 sequence is an effective inhibitor of radiolabelled VEGF binding to KDR and neuropilin-1  receptors in HUVECs and VEGF-dependent angiogenesis in an in vitro assay [ 22].	bind
39429	3	8980	7	10	NULL	0	NULL	VEGF189 	NULL		inhibits	NULL	effectively	residues 125-136 		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_4_793_s_70	12646239	A 12 amino acid peptide corresponding to residueS 125-136 of the VEGF189 sequence is an effective inhibitor of radiolabelled VEGF binding to KDR and neuropilin-1  receptors in HUVECs and VEGF-dependent angiogenesis in an in vitro assay [ 22].	bind
39431	4	8980	7	10	NULL	0	NULL	VEGF189	NULL		inhibits	NULL	effectively	residues 125-136 		statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_4_793_s_70	12646239	A 12 amino acid peptide corresponding to residueS 125-136 of the VEGF189 sequence is an effective inhibitor of radiolabelled VEGF binding to KDR and neuropilin-1  receptors in HUVECs and VEGF-dependent angiogenesis in an in vitro assay [ 22].	bind
39433	5	8980	7	NULL	NULL	0	NULL	angiogenesis	NULL		depends on	NULL				VEGF	NULL				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_4_793_s_70	12646239	A 12 amino acid peptide corresponding to residueS 125-136 of the VEGF189 sequence is an effective inhibitor of radiolabelled VEGF binding to KDR and neuropilin-1  receptors in HUVECs and VEGF-dependent angiogenesis in an in vitro assay [ 22].	bind
39435	6	8980	7	10	NULL	0	NULL	VEGF189	NULL		inhibits	NULL	effectively	residues 125-136 		statement 5	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_302_4_793_s_70	12646239	A 12 amino acid peptide corresponding to residueS 125-136 of the VEGF189 sequence is an effective inhibitor of radiolabelled VEGF binding to KDR and neuropilin-1  receptors in HUVECs and VEGF-dependent angiogenesis in an in vitro assay [ 22].	bind
30384	1	8984	6	13	NULL	NULL	NULL	Cbl protooncogene	GP		is a					120 kDa protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_5_3_197_s_123	8808675	A 120 kDa protein that binds to Grb2 has been shown to be the proto-oncogene Cbl (   Donovan et al. 1994  ; Fukazawa et al. 1995  ; Meisner et al. 1995  ).	bind
30385	2	8984	6	13	NULL	NULL	NULL	Cbl protooncogene	GP		bind					Grb2	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_5_3_197_s_123	8808675	A 120 kDa protein that binds to Grb2 has been shown to be the proto-oncogene Cbl (   Donovan et al. 1994  ; Fukazawa et al. 1995  ; Meisner et al. 1995  ).	bind
39437	1	8984	7	NULL	NULL	0	NULL	120 kDa protein	NULL		binds to	NULL				Grb2	NULL				NULL		0	NULL	NULL	NULL	gw60_immunity_5_3_197_s_123	8808675	A 120 kDa protein that binds to Grb2 has been shown to be the proto-oncogene Cbl (   Donovan et al. 1994  ; Fukazawa et al. 1995  ; Meisner et al. 1995  ).	bind
39438	2	8984	7	NULL	NULL	0	NULL	120 kDa protein	NULL		is 	NULL				 proto-oncogene Cbl	NULL				NULL		0	NULL	NULL	NULL	gw60_immunity_5_3_197_s_123	8808675	A 120 kDa protein that binds to Grb2 has been shown to be the proto-oncogene Cbl (   Donovan et al. 1994  ; Fukazawa et al. 1995  ; Meisner et al. 1995  ).	bind
30386	1	8986	6	13	NULL	NULL	NULL	UV-DDB	GP		is a 					127-kDa protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_30853_s_213	8537337	A 127-kDa Protein (UV-DDB) Binds to the Cytoplasmic Domain of the Alzheimer's Amyloid Precursor Protein.	bind
30387	2	8986	6	13	NULL	NULL	NULL	UV-DDB	GP		bind					Alzheimer's Amyloid Precursor Protein	GP		cytoplasmic domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_30853_s_213	8537337	A 127-kDa Protein (UV-DDB) Binds to the Cytoplasmic Domain of the Alzheimer's Amyloid Precursor Protein.	bind
39439	1	8986	7	10	NULL	0	NULL	UV-DDB	NULL		binds to	NULL				Alzheimer's Amyloid Precursor Protein	NULL		Cytoplasmic Domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_30853_s_213	8537337	A 127-kDa Protein (UV-DDB) Binds to the Cytoplasmic Domain of the Alzheimer's Amyloid Precursor Protein.	bind
47081	2	8986	7	10	NULL	0	NULL	UV-DDB	NULL		is	NULL				127-kDa Protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_30853_s_213	8537337	A 127-kDa Protein (UV-DDB) Binds to the Cytoplasmic Domain of the Alzheimer's Amyloid Precursor Protein.	bind
30388	1	8989	6	13	NULL	NULL	NULL	BAP-135	GP		is					135-kDa Btk-associated protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_21_11526_s_226	9326643	A 135-kDa Btk-associated protein (BAP-135) binds to the Btk PH domain ( 53).	bind
30389	2	8989	6	13	NULL	NULL	NULL	BAP-135	GP		bind					Btk	GP		PH domain		NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_21_11526_s_226	9326643	A 135-kDa Btk-associated protein (BAP-135) binds to the Btk PH domain ( 53).	bind
39441	1	8989	7	NULL	NULL	0	NULL	BAP-135	NULL		binds to	NULL				Btk	NULL		PH domain		NULL		0	NULL	NULL	NULL	gw60_pnas_94_21_11526_s_226	9326643	A 135-kDa Btk-associated protein (BAP-135) binds to the Btk PH domain ( 53).	bind
39442	2	8989	7	NULL	NULL	0	NULL	BAP-135	NULL		is	NULL				135-kDa Btk-associated protein	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_94_21_11526_s_226	9326643	A 135-kDa Btk-associated protein (BAP-135) binds to the Btk PH domain ( 53).	bind
30390	1	8990	6	13	NULL	NULL	NULL				bind			A238L		calcineurin	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_311_4_1117_s_118	14623298	A 14-amino-acid region containing the core sequence PKIIIT is both necessary and  sufficient for binding of A238L to calcineurin [ 34].	bind
47084	2	8990	6	13	NULL	NULL	NULL	14-amino-acid region	AminoAcid		contains					core sequence PKIIIT	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_311_4_1117_s_118	14623298	A 14-amino-acid region containing the core sequence PKIIIT is both necessary and  sufficient for binding of A238L to calcineurin [ 34].	bind
47085	3	8990	6	13	NULL	NULL	NULL	statement 2	Process		is necessary for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_311_4_1117_s_118	14623298	A 14-amino-acid region containing the core sequence PKIIIT is both necessary and  sufficient for binding of A238L to calcineurin [ 34].	bind
47086	4	8990	6	13	NULL	NULL	NULL	statement 2	Process		is sufficient for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_311_4_1117_s_118	14623298	A 14-amino-acid region containing the core sequence PKIIIT is both necessary and  sufficient for binding of A238L to calcineurin [ 34].	bind
39443	1	8990	7	NULL	NULL	0	NULL		NULL		bind	NULL		A238L		calcineurin	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_311_4_1117_s_118	14623298	A 14-amino-acid region containing the core sequence PKIIIT is both necessary and  sufficient for binding of A238L to calcineurin [ 34].	bind
39444	2	8990	7	10	NULL	0	NULL	14-amino-acid region	NULL		contains	NULL				core sequence PKIIIT	NULL				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_311_4_1117_s_118	14623298	A 14-amino-acid region containing the core sequence PKIIIT is both necessary and  sufficient for binding of A238L to calcineurin [ 34].	bind
47082	3	8990	7	10	NULL	0	NULL	statement 2	NULL		is necessary for	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_311_4_1117_s_118	14623298	A 14-amino-acid region containing the core sequence PKIIIT is both necessary and  sufficient for binding of A238L to calcineurin [ 34].	bind
47083	4	8990	7	10	NULL	0	NULL	statement 2	NULL		is sufficient for	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_311_4_1117_s_118	14623298	A 14-amino-acid region containing the core sequence PKIIIT is both necessary and  sufficient for binding of A238L to calcineurin [ 34].	bind
30391	1	8991	6	13	NULL	NULL	NULL	MeCP2	GP		bind					RELN	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_35_12578_s_93	16113080	A 15-day MET treatment increases MeCP2 binding to  RELN and  GAD67 promoters to an extent similar to that measured after a 6-day treatment with MET ( Fig. 3).	bind
30392	2	8991	6	13	NULL	NULL	NULL	MeCP2	GP		bind					GAD67	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_35_12578_s_93	16113080	A 15-day MET treatment increases MeCP2 binding to  RELN and  GAD67 promoters to an extent similar to that measured after a 6-day treatment with MET ( Fig. 3).	bind
30393	3	8991	6	13	NULL	NULL	NULL	MET	AminoAcid	treatment	increases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_35_12578_s_93	16113080	A 15-day MET treatment increases MeCP2 binding to  RELN and  GAD67 promoters to an extent similar to that measured after a 6-day treatment with MET ( Fig. 3).	bind
30394	4	8991	6	13	NULL	NULL	NULL	MET	AminoAcid	treatment	increases					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_35_12578_s_93	16113080	A 15-day MET treatment increases MeCP2 binding to  RELN and  GAD67 promoters to an extent similar to that measured after a 6-day treatment with MET ( Fig. 3).	bind
39479	1	8991	7	NULL	NULL	0	NULL	 MeCP2 	NULL		bind	NULL				RELN	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_pnas_102_35_12578_s_93	16113080	A 15-day MET treatment increases MeCP2 binding to  RELN and  GAD67 promoters to an extent similar to that measured after a 6-day treatment with MET ( Fig. 3).	bind
39480	2	8991	7	NULL	NULL	0	NULL	 MeCP2 	NULL		bind	NULL				GAD67	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_pnas_102_35_12578_s_93	16113080	A 15-day MET treatment increases MeCP2 binding to  RELN and  GAD67 promoters to an extent similar to that measured after a 6-day treatment with MET ( Fig. 3).	bind
39481	3	8991	7	10	NULL	0	NULL	MET	NULL	treatment	increase	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_35_12578_s_93	16113080	A 15-day MET treatment increases MeCP2 binding to  RELN and  GAD67 promoters to an extent similar to that measured after a 6-day treatment with MET ( Fig. 3).	bind
39482	4	8991	7	10	NULL	0	NULL	MET	NULL	treatment	increase	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_35_12578_s_93	16113080	A 15-day MET treatment increases MeCP2 binding to  RELN and  GAD67 promoters to an extent similar to that measured after a 6-day treatment with MET ( Fig. 3).	bind
30395	1	8992	6	13	NULL	NULL	NULL	hnRNP	GP		bind				E1 region	alpha-globin RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_48_49680_s_249	15364910	A 15-lipoxygenase differentiation control element sequence also serves as the minimal binding element for binding of hnRNPs E1 and E2 to alpha-globin RNA ( ).	bind
30396	2	8992	6	13	NULL	NULL	NULL	hnRNP 	GP		bind				E2 region	alpha-globin RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_48_49680_s_249	15364910	A 15-lipoxygenase differentiation control element sequence also serves as the minimal binding element for binding of hnRNPs E1 and E2 to alpha-globin RNA ( ).	bind
31158	3	8992	6	13	NULL	NULL	NULL	15-lipoxygenase	GP	sequence of	serves as				differentiation control element					minimal binding element	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_48_49680_s_249	15364910	A 15-lipoxygenase differentiation control element sequence also serves as the minimal binding element for binding of hnRNPs E1 and E2 to alpha-globin RNA ( ).	bind
31159	4	8992	6	13	NULL	NULL	NULL	statement 3	GP		occurs for					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_48_49680_s_249	15364910	A 15-lipoxygenase differentiation control element sequence also serves as the minimal binding element for binding of hnRNPs E1 and E2 to alpha-globin RNA ( ).	bind
31160	5	8992	6	13	NULL	NULL	NULL	statement 3	GP		occurs for					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_48_49680_s_249	15364910	A 15-lipoxygenase differentiation control element sequence also serves as the minimal binding element for binding of hnRNPs E1 and E2 to alpha-globin RNA ( ).	bind
39483	1	8992	7	NULL	NULL	0	NULL	hnRNPs E1	NULL		bind	NULL				alpha-globin RNA	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_49680_s_249	15364910	A 15-lipoxygenase differentiation control element sequence also serves as the minimal binding element for binding of hnRNPs E1 and E2 to alpha-globin RNA ( ).	bind
39484	2	8992	7	NULL	NULL	0	NULL	hnRNPs E2	NULL		bind	NULL				alpha-globin RNA	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_49680_s_249	15364910	A 15-lipoxygenase differentiation control element sequence also serves as the minimal binding element for binding of hnRNPs E1 and E2 to alpha-globin RNA ( ).	bind
39485	3	8992	7	NULL	NULL	0	NULL	15-lipoxygenase	NULL		serve as	NULL			differentiation control element sequence	minimal binding element	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_49680_s_249	15364910	A 15-lipoxygenase differentiation control element sequence also serves as the minimal binding element for binding of hnRNPs E1 and E2 to alpha-globin RNA ( ).	bind
39486	4	8992	7	NULL	NULL	0	NULL	statement 3	NULL		is required for	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_49680_s_249	15364910	A 15-lipoxygenase differentiation control element sequence also serves as the minimal binding element for binding of hnRNPs E1 and E2 to alpha-globin RNA ( ).	bind
39487	5	8992	7	NULL	NULL	0	NULL	statement 3	NULL		is required for	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_49680_s_249	15364910	A 15-lipoxygenase differentiation control element sequence also serves as the minimal binding element for binding of hnRNPs E1 and E2 to alpha-globin RNA ( ).	bind
40393	1	8995	6	13	NULL	NULL	NULL	Arg1	GP		contains				promoter					STAT6 binding site	NULL		NULL	NULL	NULL	NULL	gw70_gene_353_1_98_s_29	15922518	A 150-bp region containing  the STAT6 and CEBP binding site was created by PCR amplification of the  2850 to   2999 region of the Arg1 promoter and cloned into the  HindIII/ XhoI sites just upstream of the 81-bp thymidine kinase promoter in the pT81-luc reporter  plasmid (  Nordeen, 1988) to create IL4RE-pT81-luc.	bind
40394	2	8995	6	13	NULL	NULL	NULL	Arg1	GP		contains				promoter					CEBP binding site	NULL		NULL	NULL	NULL	NULL	gw70_gene_353_1_98_s_29	15922518	A 150-bp region containing  the STAT6 and CEBP binding site was created by PCR amplification of the  2850 to   2999 region of the Arg1 promoter and cloned into the  HindIII/ XhoI sites just upstream of the 81-bp thymidine kinase promoter in the pT81-luc reporter  plasmid (  Nordeen, 1988) to create IL4RE-pT81-luc.	bind
40401	1	8995	7	10	NULL	0	NULL	Arg1	NULL		contains	NULL			 promoter		NULL			STAT6 binding site	NULL		NULL	NULL	NULL	NULL	gw70_gene_353_1_98_s_29	15922518	A 150-bp region containing  the STAT6 and CEBP binding site was created by PCR amplification of the  2850 to   2999 region of the Arg1 promoter and cloned into the  HindIII/ XhoI sites just upstream of the 81-bp thymidine kinase promoter in the pT81-luc reporter  plasmid (  Nordeen, 1988) to create IL4RE-pT81-luc.	bind
40402	2	8995	7	10	NULL	0	NULL	Arg1	NULL		contains	NULL			promoter		NULL			CEBP binding site	NULL		NULL	NULL	NULL	NULL	gw70_gene_353_1_98_s_29	15922518	A 150-bp region containing  the STAT6 and CEBP binding site was created by PCR amplification of the  2850 to   2999 region of the Arg1 promoter and cloned into the  HindIII/ XhoI sites just upstream of the 81-bp thymidine kinase promoter in the pT81-luc reporter  plasmid (  Nordeen, 1988) to create IL4RE-pT81-luc.	bind
30398	1	8996	6	13	NULL	NULL	NULL	adhesin	GP	Porphyromonas (Bacteroides) gingivalis	bind					fibrinogen	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_9_5218_s_226	10948147	A 150-kDa fibrinogen binding adhesin of  Porphyromonas (Bacteroides) gingivalis also recognized fibronectin ( 9,  10).	bind
30399	2	8996	6	13	NULL	NULL	NULL	adhesin	GP	Porphyromonas (Bacteroides) gingivalis	is					150-kDa protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_9_5218_s_226	10948147	A 150-kDa fibrinogen binding adhesin of  Porphyromonas (Bacteroides) gingivalis also recognized fibronectin ( 9,  10).	bind
30400	3	8996	6	13	NULL	NULL	NULL	adhesion	GP	Porphyromonas (Bacteroides) gingivalis	recognize					fibronectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_9_5218_s_226	10948147	A 150-kDa fibrinogen binding adhesin of  Porphyromonas (Bacteroides) gingivalis also recognized fibronectin ( 9,  10).	bind
39488	1	8996	7	10	NULL	0	NULL	adhesin	NULL	Porphyromonas  gingivalis 	recognize	NULL		 		fibronectin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_9_5218_s_226	10948147	A 150-kDa fibrinogen binding adhesin of  Porphyromonas (Bacteroides) gingivalis also recognized fibronectin ( 9,  10).	bind
39489	2	8996	7	NULL	NULL	0	NULL	Porphyromonas gingivalis 	NULL		is a type of	NULL				Bacteroides	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_9_5218_s_226	10948147	A 150-kDa fibrinogen binding adhesin of  Porphyromonas (Bacteroides) gingivalis also recognized fibronectin ( 9,  10).	bind
47091	3	8996	7	10	NULL	0	NULL	adhesin	NULL	Porphyromonas gingivalis 	bind	NULL				fibrinogen	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_9_5218_s_226	10948147	A 150-kDa fibrinogen binding adhesin of  Porphyromonas (Bacteroides) gingivalis also recognized fibronectin ( 9,  10).	bind
47092	4	8996	7	10	NULL	0	NULL	adhesin	NULL	\tPorphyromonas gingivalis 	is	NULL				150-kDa protein	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_9_5218_s_226	10948147	A 150-kDa fibrinogen binding adhesin of  Porphyromonas (Bacteroides) gingivalis also recognized fibronectin ( 9,  10).	bind
30401	1	8997	6	13	NULL	NULL	NULL	150-kDa surface component	GP	P. gingivalis	bind					fibrinogen	GP				NULL		NULL	NULL	NULL	NULL	gw60_annurevmicrobiol_50_0_513_s_346	8905090	A 150-kDa surface component of  P. gingivalis binds to  fibrinogen ( 131).	bind
39490	1	8997	7	10	NULL	0	NULL	150-kDa surface component 	NULL	P. gingivalis	binds to	NULL				fibrinogen	NULL				NULL		NULL	NULL	NULL	NULL	gw60_annurevmicrobiol_50_0_513_s_346	8905090	A 150-kDa surface component of  P. gingivalis binds to  fibrinogen ( 131).	bind
30402	1	8998	6	13	NULL	NULL	NULL	155-kDa protein	GP		is a subunit of		largest			pol III	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_14_7795_s_90	11416169	A 155-kDa protein, which was identified subsequently as the largest subunit of pol III by immunoblot analysis using RPC155-specific antibodies (lane 3), binds plakophilin 2 selectively.	bind
30403	2	8998	6	13	NULL	NULL	NULL	statement 1	GP		bind		selectively			plakophilin 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_14_7795_s_90	11416169	A 155-kDa protein, which was identified subsequently as the largest subunit of pol III by immunoblot analysis using RPC155-specific antibodies (lane 3), binds plakophilin 2 selectively.	bind
39491	1	8998	7	NULL	NULL	0	NULL	pol III	NULL		binds	NULL	selectively	155-kDa protein subunit		plakophilin 2 	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_98_14_7795_s_90	11416169	A 155-kDa protein, which was identified subsequently as the largest subunit of pol III by immunoblot analysis using RPC155-specific antibodies (lane 3), binds plakophilin 2 selectively.	bind
30404	1	8999	6	13	NULL	NULL	NULL	16-mer peptide	GP		represents					BAD	GP	bona fide	BH3 domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_25_17321_s_400	16603546	A 16-mer peptide representing the  bona fide BH3 domain of BAD bound Bcl-XL only poorly.	bind
30405	2	8999	6	13	NULL	NULL	NULL	BAD	GP		bind		poorly	BH3 domain		BCL-XL	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_25_17321_s_400	16603546	A 16-mer peptide representing the  bona fide BH3 domain of BAD bound Bcl-XL only poorly.	bind
39492	1	8999	7	10	NULL	0	NULL	BAD	NULL		binds	NULL	poorly	BH3 domain 		Bcl-XL	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_25_17321_s_400	16603546	A 16-mer peptide representing the  bona fide BH3 domain of BAD bound Bcl-XL only poorly.	bind
47090	2	8999	7	10	NULL	0	NULL	16-mer peptide	NULL		represents	NULL				BAD	NULL	bona fide	BH3 domain		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_25_17321_s_400	16603546	A 16-mer peptide representing the  bona fide BH3 domain of BAD bound Bcl-XL only poorly.	bind
38584	1	9001	5	11	NULL	NULL	NULL	160-kDa protein	GP		bind					Shc	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_25_23097_s_202	11312266	A 160-kDa protein that co-immunoprecipitated with Shc also showed increased tyrosine phosphorylation in response to p75NTR overexpression; this protein is likely SHIP, a 160-kDa lipid phosphatase that binds activated Shc with high affinity ( 53).	bind
38585	3	9001	5	11	NULL	NULL	NULL	p75NTR	GP	overexpression of	increase					SHIP	GP	phosphorylation of	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_25_23097_s_202	11312266	A 160-kDa protein that co-immunoprecipitated with Shc also showed increased tyrosine phosphorylation in response to p75NTR overexpression; this protein is likely SHIP, a 160-kDa lipid phosphatase that binds activated Shc with high affinity ( 53).	bind
38711	4	9001	5	11	NULL	NULL	NULL	SHIP	GP		bind		high affinity			Shc	GP	activated			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_25_23097_s_202	11312266	A 160-kDa protein that co-immunoprecipitated with Shc also showed increased tyrosine phosphorylation in response to p75NTR overexpression; this protein is likely SHIP, a 160-kDa lipid phosphatase that binds activated Shc with high affinity ( 53).	bind
39020	2	9001	5	11	NULL	NULL	NULL	160-kDa protein	GP		is					SHIP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_25_23097_s_202	11312266	A 160-kDa protein that co-immunoprecipitated with Shc also showed increased tyrosine phosphorylation in response to p75NTR overexpression; this protein is likely SHIP, a 160-kDa lipid phosphatase that binds activated Shc with high affinity ( 53).	bind
39021	5	9001	5	11	NULL	NULL	NULL	SHIP	GP		is a type of					lipid phosphatase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_25_23097_s_202	11312266	A 160-kDa protein that co-immunoprecipitated with Shc also showed increased tyrosine phosphorylation in response to p75NTR overexpression; this protein is likely SHIP, a 160-kDa lipid phosphatase that binds activated Shc with high affinity ( 53).	bind
31161	1	9001	6	11	NULL	NULL	NULL	160-kDa protein	GP		bind					Shc	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_25_23097_s_202	11312266	A 160-kDa protein that co-immunoprecipitated with Shc also showed increased tyrosine phosphorylation in response to p75NTR overexpression; this protein is likely SHIP, a 160-kDa lipid phosphatase that binds activated Shc with high affinity ( 53).	bind
31162	2	9001	6	11	NULL	NULL	NULL	160-kDa protein	GP		is phosphorylated on								tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_25_23097_s_202	11312266	A 160-kDa protein that co-immunoprecipitated with Shc also showed increased tyrosine phosphorylation in response to p75NTR overexpression; this protein is likely SHIP, a 160-kDa lipid phosphatase that binds activated Shc with high affinity ( 53).	bind
31163	3	9001	6	11	NULL	NULL	NULL	statement 2	Process		occurs in response to					p75NTR	GP	overexpression of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_25_23097_s_202	11312266	A 160-kDa protein that co-immunoprecipitated with Shc also showed increased tyrosine phosphorylation in response to p75NTR overexpression; this protein is likely SHIP, a 160-kDa lipid phosphatase that binds activated Shc with high affinity ( 53).	bind
31164	4	9001	6	11	NULL	NULL	NULL	160-kDa protein	GP		is 		probably			SHIP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_25_23097_s_202	11312266	A 160-kDa protein that co-immunoprecipitated with Shc also showed increased tyrosine phosphorylation in response to p75NTR overexpression; this protein is likely SHIP, a 160-kDa lipid phosphatase that binds activated Shc with high affinity ( 53).	bind
31165	5	9001	6	11	NULL	NULL	NULL	SHIP	GP		is a type of					lipid phosphatase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_25_23097_s_202	11312266	A 160-kDa protein that co-immunoprecipitated with Shc also showed increased tyrosine phosphorylation in response to p75NTR overexpression; this protein is likely SHIP, a 160-kDa lipid phosphatase that binds activated Shc with high affinity ( 53).	bind
31166	6	9001	6	11	NULL	NULL	NULL	SHIP	GP		bind		high affinity			Shc	GP	activated			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_25_23097_s_202	11312266	A 160-kDa protein that co-immunoprecipitated with Shc also showed increased tyrosine phosphorylation in response to p75NTR overexpression; this protein is likely SHIP, a 160-kDa lipid phosphatase that binds activated Shc with high affinity ( 53).	bind
49154	1	9002	5	11	NULL	NULL	NULL	p HP0294 probe	NucleicAcid		does not bind					HP0166-His6 protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_5_1750_s_125	16484186	A 161-bp probe for p HP0294 ( amiE) that did not bind to HP0166-His6 protein under the same experimental condition is shown in Fig.  2B to serve as a negative (nonspecific) control.	bind
30406	1	9002	6	11	NULL	NULL	NULL	p HP0294 probe	NucleicAcid		does not bind					HP0166-His6 protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_5_1750_s_125	16484186	A 161-bp probe for p HP0294 ( amiE) that did not bind to HP0166-His6 protein under the same experimental condition is shown in Fig.  2B to serve as a negative (nonspecific) control.	bind
38591	2	9005	5	11	NULL	NULL	NULL	statement1	AminoAcid		does not bind					RNAs	NucleicAcid	capped			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_30551_s_122	10887196	A 17-amino acid peptide comprising the minimal eIF4E binding motif of eIF4G failed to produce any shift with capped RNAs.	bind
47907	1	9005	5	11	NULL	NULL	NULL	17-amino acid peptide 	AminoAcid		comprise					eIF4G	GP		minimal eIF4E binding motif   		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_30551_s_122	10887196	A 17-amino acid peptide comprising the minimal eIF4E binding motif of eIF4G failed to produce any shift with capped RNAs.	bind
31167	2	9005	6	11	NULL	NULL	NULL	statement 1	AminoAcid		does not bind					 RNA	NucleicAcid	capped			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_30551_s_122	10887196	A 17-amino acid peptide comprising the minimal eIF4E binding motif of eIF4G failed to produce any shift with capped RNAs.	bind
47908	1	9005	6	11	NULL	NULL	NULL	17-amino acid peptide 	AminoAcid		comprise					eIF4G	GP		minimal eIF4E binding motif 		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_30551_s_122	10887196	A 17-amino acid peptide comprising the minimal eIF4E binding motif of eIF4G failed to produce any shift with capped RNAs.	bind
38592	1	9006	5	11	NULL	NULL	NULL	170-kD APN	GP		bind		high affinity			Cry1A toxins	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5531_857_s_43	11486086	A 170-kD APN (Receptor A) binds Cry1A toxins with high affinity and mediates Bt toxin-induced pore formation when reconstituted into phospholipid vesicles in vitro ( 7).	bind
38593	2	9006	5	11	NULL	NULL	NULL	Bt toxin	Chemical		induce					pore	CellComponent	formation of			NULL		NULL	NULL	NULL	NULL	gw60_science_293_5531_857_s_43	11486086	A 170-kD APN (Receptor A) binds Cry1A toxins with high affinity and mediates Bt toxin-induced pore formation when reconstituted into phospholipid vesicles in vitro ( 7).	bind
38594	3	9006	5	11	NULL	NULL	NULL	statement 1	Process		mediate					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5531_857_s_43	11486086	A 170-kD APN (Receptor A) binds Cry1A toxins with high affinity and mediates Bt toxin-induced pore formation when reconstituted into phospholipid vesicles in vitro ( 7).	bind
38595	4	9006	5	11	NULL	NULL	NULL	170-kD APN	GP		is reconstituted into					phospholipid vesicles	CellComponent				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_science_293_5531_857_s_43	11486086	A 170-kD APN (Receptor A) binds Cry1A toxins with high affinity and mediates Bt toxin-induced pore formation when reconstituted into phospholipid vesicles in vitro ( 7).	bind
38596	5	9006	5	11	NULL	NULL	NULL	statement 4	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5531_857_s_43	11486086	A 170-kD APN (Receptor A) binds Cry1A toxins with high affinity and mediates Bt toxin-induced pore formation when reconstituted into phospholipid vesicles in vitro ( 7).	bind
57752	6	9006	5	11	NULL	NULL	NULL	APN	GP		is a type of					Receptor A	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5531_857_s_43	11486086	A 170-kD APN (Receptor A) binds Cry1A toxins with high affinity and mediates Bt toxin-induced pore formation when reconstituted into phospholipid vesicles in vitro ( 7).	bind
30407	1	9006	6	11	NULL	NULL	NULL	170-kD APN	GP		bind		high affinity			Cry1A toxins	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5531_857_s_43	11486086	A 170-kD APN (Receptor A) binds Cry1A toxins with high affinity and mediates Bt toxin-induced pore formation when reconstituted into phospholipid vesicles in vitro ( 7).	bind
30408	2	9006	6	11	NULL	NULL	NULL	Bt toxin	Chemical		induces					pore	CellComponent	formation of 			NULL		NULL	NULL	NULL	NULL	gw60_science_293_5531_857_s_43	11486086	A 170-kD APN (Receptor A) binds Cry1A toxins with high affinity and mediates Bt toxin-induced pore formation when reconstituted into phospholipid vesicles in vitro ( 7).	bind
30409	3	9006	6	11	NULL	NULL	NULL	APN	GP		is a type of					receptor A	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5531_857_s_43	11486086	A 170-kD APN (Receptor A) binds Cry1A toxins with high affinity and mediates Bt toxin-induced pore formation when reconstituted into phospholipid vesicles in vitro ( 7).	bind
30410	4	9006	6	11	NULL	NULL	NULL	statement 1	Process		mediates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5531_857_s_43	11486086	A 170-kD APN (Receptor A) binds Cry1A toxins with high affinity and mediates Bt toxin-induced pore formation when reconstituted into phospholipid vesicles in vitro ( 7).	bind
30411	5	9006	6	11	NULL	NULL	NULL	170-kD APN	GP		is reconstituted into					phospholipid vesicles	CellComponent				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_science_293_5531_857_s_43	11486086	A 170-kD APN (Receptor A) binds Cry1A toxins with high affinity and mediates Bt toxin-induced pore formation when reconstituted into phospholipid vesicles in vitro ( 7).	bind
30412	6	9006	6	11	NULL	NULL	NULL	statement 4	Process		occurs via					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5531_857_s_43	11486086	A 170-kD APN (Receptor A) binds Cry1A toxins with high affinity and mediates Bt toxin-induced pore formation when reconstituted into phospholipid vesicles in vitro ( 7).	bind
38769	1	9009	5	11	NULL	NULL	NULL	SARS coronavirus S protein 	GP		bind		efficiently	193-amino acid fragment		angiotensin-converting enzyme 2	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-biol-chem_279_5_14670965_s_1	14670965	A 193-amino acid fragment of the SARS coronavirus S protein efficiently binds angiotensin-converting enzyme 2..	bind
30413	1	9009	6	11	NULL	NULL	NULL	SARS coronavirus S protein	GP		bind		efficiently	193-amino acid fragment		angiotensin-converting enzyme 2	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-biol-chem_279_5_14670965_s_1	14670965	A 193-amino acid fragment of the SARS coronavirus S protein efficiently binds angiotensin-converting enzyme 2..	bind
38770	1	9011	5	11	NULL	NULL	NULL	fimbrin	GP		interact with					vimentin subunit	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_146_4_831_s_11	10459017	A 1:4 stoichiometry of fimbrin binding to vimentin and a low percentage (1%) of the extracted vimentin suggest that fimbrin interacts with a vimentin subunit.	bind
38771	2	9011	5	11	NULL	NULL	NULL	fimbrin	GP		bind					vimentin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_146_4_831_s_11	10459017	A 1:4 stoichiometry of fimbrin binding to vimentin and a low percentage (1%) of the extracted vimentin suggest that fimbrin interacts with a vimentin subunit.	bind
31168	1	9011	6	11	NULL	NULL	NULL	fimbrin	GP		interacts with					vimentin subunit	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_146_4_831_s_11	10459017	A 1:4 stoichiometry of fimbrin binding to vimentin and a low percentage (1%) of the extracted vimentin suggest that fimbrin interacts with a vimentin subunit.	bind
47909	2	9011	6	11	NULL	NULL	NULL	fimbrin	GP		bind					vimentin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_146_4_831_s_11	10459017	A 1:4 stoichiometry of fimbrin binding to vimentin and a low percentage (1%) of the extracted vimentin suggest that fimbrin interacts with a vimentin subunit.	bind
38772	1	9012	5	11	NULL	NULL	NULL	RNA aptamer	NucleicAcid		bind					hnps-PLA2	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevmed_56_0_555_s_231	15660527	A 2''-fluoropyrimidine-modified RNA selection against hnps-PLA2 ( 65) isolated an RNA aptamer that binds to hnps-PLA2 with a Kd of 1.7 nM and inhibits hnps-PLA2 activity with an IC50 of 4 nM.	bind
38774	2	9012	5	11	NULL	NULL	NULL	statement 1	GP		inhibit					hnps-PLA2	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw70_annurevmed_56_0_555_s_231	15660527	A 2''-fluoropyrimidine-modified RNA selection against hnps-PLA2 ( 65) isolated an RNA aptamer that binds to hnps-PLA2 with a Kd of 1.7 nM and inhibits hnps-PLA2 activity with an IC50 of 4 nM.	bind
30445	1	9012	6	11	NULL	NULL	NULL	RNA aptamer 	NucleicAcid		bind					hnps-PLA2	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevmed_56_0_555_s_231	15660527	A 2''-fluoropyrimidine-modified RNA selection against hnps-PLA2 ( 65) isolated an RNA aptamer that binds to hnps-PLA2 with a Kd of 1.7 nM and inhibits hnps-PLA2 activity with an IC50 of 4 nM.	bind
30446	2	9012	6	11	NULL	NULL	NULL	RNA aptamer	NucleicAcid		inhibits					hnps-PLA2	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw70_annurevmed_56_0_555_s_231	15660527	A 2''-fluoropyrimidine-modified RNA selection against hnps-PLA2 ( 65) isolated an RNA aptamer that binds to hnps-PLA2 with a Kd of 1.7 nM and inhibits hnps-PLA2 activity with an IC50 of 4 nM.	bind
38777	1	9013	5	11	NULL	NULL	NULL	DRIP205	GP		bind					VDR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2718_s_142	10733574	A 2- to 20-fold molar excess of NR2 peptide over DRIP205 was able to efficiently compete DRIP205 binding to VDR, but the same ratio of NR1 peptide or an unrelated nonspecific peptide was unable to compete for this interaction (Fig.  4B, compare lanes 5 to 7 to lanes 2 to 4 or 8 to 10).	bind
38779	2	9013	5	11	NULL	NULL	NULL	NR2 peptide	GP		bind					VDR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2718_s_142	10733574	A 2- to 20-fold molar excess of NR2 peptide over DRIP205 was able to efficiently compete DRIP205 binding to VDR, but the same ratio of NR1 peptide or an unrelated nonspecific peptide was unable to compete for this interaction (Fig.  4B, compare lanes 5 to 7 to lanes 2 to 4 or 8 to 10).	bind
38780	3	9013	5	11	NULL	NULL	NULL	statement 2	Process		competes with		efficiently			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2718_s_142	10733574	A 2- to 20-fold molar excess of NR2 peptide over DRIP205 was able to efficiently compete DRIP205 binding to VDR, but the same ratio of NR1 peptide or an unrelated nonspecific peptide was unable to compete for this interaction (Fig.  4B, compare lanes 5 to 7 to lanes 2 to 4 or 8 to 10).	bind
38781	4	9013	5	11	NULL	NULL	NULL	NR1 peptide	GP		does not compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2718_s_142	10733574	A 2- to 20-fold molar excess of NR2 peptide over DRIP205 was able to efficiently compete DRIP205 binding to VDR, but the same ratio of NR1 peptide or an unrelated nonspecific peptide was unable to compete for this interaction (Fig.  4B, compare lanes 5 to 7 to lanes 2 to 4 or 8 to 10).	bind
30448	1	9013	6	11	NULL	NULL	NULL	DRIP205	GP		bind					VDR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2718_s_142	10733574	A 2- to 20-fold molar excess of NR2 peptide over DRIP205 was able to efficiently compete DRIP205 binding to VDR, but the same ratio of NR1 peptide or an unrelated nonspecific peptide was unable to compete for this interaction (Fig.  4B, compare lanes 5 to 7 to lanes 2 to 4 or 8 to 10).	bind
30449	2	9013	6	11	NULL	NULL	NULL	NR2 peptide	GP	excess of	bind					VDR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2718_s_142	10733574	A 2- to 20-fold molar excess of NR2 peptide over DRIP205 was able to efficiently compete DRIP205 binding to VDR, but the same ratio of NR1 peptide or an unrelated nonspecific peptide was unable to compete for this interaction (Fig.  4B, compare lanes 5 to 7 to lanes 2 to 4 or 8 to 10).	bind
30450	3	9013	6	11	NULL	NULL	NULL	statement 1	Process		competes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2718_s_142	10733574	A 2- to 20-fold molar excess of NR2 peptide over DRIP205 was able to efficiently compete DRIP205 binding to VDR, but the same ratio of NR1 peptide or an unrelated nonspecific peptide was unable to compete for this interaction (Fig.  4B, compare lanes 5 to 7 to lanes 2 to 4 or 8 to 10).	bind
30451	4	9013	6	11	NULL	NULL	NULL	NR1 peptide	GP	excess of	does not bind					VDR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2718_s_142	10733574	A 2- to 20-fold molar excess of NR2 peptide over DRIP205 was able to efficiently compete DRIP205 binding to VDR, but the same ratio of NR1 peptide or an unrelated nonspecific peptide was unable to compete for this interaction (Fig.  4B, compare lanes 5 to 7 to lanes 2 to 4 or 8 to 10).	bind
38785	1	9014	5	11	NULL	NULL	NULL	alpha-Gal-(1,3)-beta-Gal-(1,4)-beta-GlcNAcO(CH(2))(8)CO(2)CH(3)	Chemical	extended conformation	bind					TcdA	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_nat-struct-mol-biol_13_5_16622409_s_3	16622409	A 2-A resolution cocrystal structure reveals  two molecules of alpha-Gal-(1,3)-beta-Gal-(1,4)-beta-GlcNAcO(CH(2))(8)CO(2)CH(3)  binding in an extended conformation to TcdA.	bind
30452	1	9014	6	11	NULL	NULL	NULL	alpha-Gal-(1,3)-beta-Gal-(1,4)-beta-GlcNAcO(CH(2))(8)CO(2)CH(3)	Chemical	extended conformation of	bind					TcdA	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_nat-struct-mol-biol_13_5_16622409_s_3	16622409	A 2-A resolution cocrystal structure reveals  two molecules of alpha-Gal-(1,3)-beta-Gal-(1,4)-beta-GlcNAcO(CH(2))(8)CO(2)CH(3)  binding in an extended conformation to TcdA.	bind
38787	1	9015	5	11	NULL	NULL	NULL	BF-1	GP		bind					double-stranded DNA	NucleicAcid			high-affinity site	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6201_s_310	10938097	A 2-amino-acid mutation (NH-AA) within the third alpha-helix of the WH domain abolishes the ability of BF-1 to bind to a high-affinity site on double-stranded DNA.	bind
38789	2	9015	5	11	NULL	NULL	NULL	BF-1	GP	mutant	abolishes			(NH-AA) within the third alpha-helix of WH domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6201_s_310	10938097	A 2-amino-acid mutation (NH-AA) within the third alpha-helix of the WH domain abolishes the ability of BF-1 to bind to a high-affinity site on double-stranded DNA.	bind
38790	3	9015	5	11	NULL	NULL	NULL	NH-AA	Chemical		is					2-amino-acid mutation	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6201_s_310	10938097	A 2-amino-acid mutation (NH-AA) within the third alpha-helix of the WH domain abolishes the ability of BF-1 to bind to a high-affinity site on double-stranded DNA.	bind
30453	1	9015	6	11	NULL	NULL	NULL	BF-1	GP		bind					double-stranded DNA	NucleicAcid			high-affinity site	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6201_s_310	10938097	A 2-amino-acid mutation (NH-AA) within the third alpha-helix of the WH domain abolishes the ability of BF-1 to bind to a high-affinity site on double-stranded DNA.	bind
30454	2	9015	6	11	NULL	NULL	NULL	BF-1	GP	mutant	abolishes			NH-AA within third alpha-helix of the WH domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6201_s_310	10938097	A 2-amino-acid mutation (NH-AA) within the third alpha-helix of the WH domain abolishes the ability of BF-1 to bind to a high-affinity site on double-stranded DNA.	bind
47910	3	9015	6	11	NULL	NULL	NULL	NH-AA	Chemical		is					2-amino-acid mutation 	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6201_s_310	10938097	A 2-amino-acid mutation (NH-AA) within the third alpha-helix of the WH domain abolishes the ability of BF-1 to bind to a high-affinity site on double-stranded DNA.	bind
38791	1	9016	5	13	NULL	NULL	NULL	CRP	GP	induced	bind					RBC(Mal)	Cell				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_glycoconj-j_23_3-4_16691506_s_8	16691506	A 2.3-fold increased binding of induced CRP to RBC(Mal) as  compared to normal erythrocytes (RBC(N)) confirmed disease-specificity.	bind
38795	3	9016	5	13	NULL	NULL	NULL	statement 1	Process	increased	confirms					disease-specificity	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_glycoconj-j_23_3-4_16691506_s_8	16691506	A 2.3-fold increased binding of induced CRP to RBC(Mal) as  compared to normal erythrocytes (RBC(N)) confirmed disease-specificity.	bind
47911	2	9016	5	13	NULL	NULL	NULL	CRP	GP	induced	bind					erythrocytes 	Cell	normal			NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_glycoconj-j_23_3-4_16691506_s_8	16691506	A 2.3-fold increased binding of induced CRP to RBC(Mal) as  compared to normal erythrocytes (RBC(N)) confirmed disease-specificity.	bind
47912	4	9016	5	13	NULL	NULL	NULL	RBC(N)	Cell		is					normal erythrocytes	Cell				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_glycoconj-j_23_3-4_16691506_s_8	16691506	A 2.3-fold increased binding of induced CRP to RBC(Mal) as  compared to normal erythrocytes (RBC(N)) confirmed disease-specificity.	bind
30455	1	9016	6	NULL	NULL	0	NULL	CRP	NULL	induced	bind	NULL				RBC(Mal)	NULL				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_glycoconj-j_23_3-4_16691506_s_8	16691506	A 2.3-fold increased binding of induced CRP to RBC(Mal) as  compared to normal erythrocytes (RBC(N)) confirmed disease-specificity.	bind
30456	2	9016	6	NULL	NULL	0	NULL	CRP	NULL	induced	bind	NULL				erythrocytes	NULL	normal			NULL		0	NULL	NULL	NULL	abs-batch0680-0699_glycoconj-j_23_3-4_16691506_s_8	16691506	A 2.3-fold increased binding of induced CRP to RBC(Mal) as  compared to normal erythrocytes (RBC(N)) confirmed disease-specificity.	bind
30457	3	9016	6	NULL	NULL	0	NULL	RBC(N)	NULL		is	NULL				normal erythrocytes	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_glycoconj-j_23_3-4_16691506_s_8	16691506	A 2.3-fold increased binding of induced CRP to RBC(Mal) as  compared to normal erythrocytes (RBC(N)) confirmed disease-specificity.	bind
47913	4	9016	6	10	NULL	0	NULL	statement 1	NULL	increased	confirms	NULL				disease-specificity	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_glycoconj-j_23_3-4_16691506_s_8	16691506	A 2.3-fold increased binding of induced CRP to RBC(Mal) as  compared to normal erythrocytes (RBC(N)) confirmed disease-specificity.	bind
38800	2	9017	5	13	NULL	NULL	NULL	HMG-1	GP		complex with			box A		statement 1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_33	10825199	A 2.5- Ang  crystal structure of the HMG-1 box A complexed to cisplatin-modified DNA reveals that DNA binding by HMG-1 shares many features with that of LEF-1 ( 40).	bind
47914	1	9017	5	13	NULL	NULL	NULL	cisplatin	Chemical		modifies					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_33	10825199	A 2.5- Ang  crystal structure of the HMG-1 box A complexed to cisplatin-modified DNA reveals that DNA binding by HMG-1 shares many features with that of LEF-1 ( 40).	bind
47915	3	9017	5	13	NULL	NULL	NULL	statement 1	Process		shares features with					LEF-1	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_33	10825199	A 2.5- Ang  crystal structure of the HMG-1 box A complexed to cisplatin-modified DNA reveals that DNA binding by HMG-1 shares many features with that of LEF-1 ( 40).	bind
30559	2	9017	6	10	NULL	0	NULL	HMG-1	NULL		complex with	NULL		box A		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_33	10825199	A 2.5- Ang  crystal structure of the HMG-1 box A complexed to cisplatin-modified DNA reveals that DNA binding by HMG-1 shares many features with that of LEF-1 ( 40).	bind
30563	3	9017	6	10	NULL	0	NULL	statement 1	NULL		shares features with	NULL				LEF-1	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_33	10825199	A 2.5- Ang  crystal structure of the HMG-1 box A complexed to cisplatin-modified DNA reveals that DNA binding by HMG-1 shares many features with that of LEF-1 ( 40).	bind
47916	1	9017	6	10	NULL	0	NULL	cisplatin	NULL		modifies	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_12_4359_s_33	10825199	A 2.5- Ang  crystal structure of the HMG-1 box A complexed to cisplatin-modified DNA reveals that DNA binding by HMG-1 shares many features with that of LEF-1 ( 40).	bind
38815	1	9018	5	13	NULL	NULL	NULL	importin beta	GP		bind					AhR complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_4_2677_s_210	12431985	A 2.5-fold increase in binding of importin beta to the AhR complex was detected relative to background binding.	bind
30566	1	9018	6	NULL	NULL	0	NULL	importin beta	NULL		bind	NULL				AhR complex	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_4_2677_s_210	12431985	A 2.5-fold increase in binding of importin beta to the AhR complex was detected relative to background binding.	bind
38812	1	9019	5	13	NULL	NULL	NULL	p53	GP		bind					PIG3	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_10_3375_s_232	11313463	A 2.5-fold increase in p53 binding to the PIG3 promoter was observed by 4 h after ADR treatment (Fig.  2C); and although this increase in binding was accompanied by an increase in PIG3 mRNA, it was modest at 1.5-fold of the control level (Fig.  5A and B).	bind
38813	2	9019	5	13	NULL	NULL	NULL	ADR	Chemical	treatment	increase					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_10_3375_s_232	11313463	A 2.5-fold increase in p53 binding to the PIG3 promoter was observed by 4 h after ADR treatment (Fig.  2C); and although this increase in binding was accompanied by an increase in PIG3 mRNA, it was modest at 1.5-fold of the control level (Fig.  5A and B).	bind
38814	3	9019	5	13	NULL	NULL	NULL	statement 2	Process		is accompanied by					PIG3 mRNA	NucleicAcid	increase in			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_10_3375_s_232	11313463	A 2.5-fold increase in p53 binding to the PIG3 promoter was observed by 4 h after ADR treatment (Fig.  2C); and although this increase in binding was accompanied by an increase in PIG3 mRNA, it was modest at 1.5-fold of the control level (Fig.  5A and B).	bind
30567	1	9019	6	NULL	NULL	0	NULL	p53	NULL		bind	NULL				PIG3	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_10_3375_s_232	11313463	A 2.5-fold increase in p53 binding to the PIG3 promoter was observed by 4 h after ADR treatment (Fig.  2C); and although this increase in binding was accompanied by an increase in PIG3 mRNA, it was modest at 1.5-fold of the control level (Fig.  5A and B).	bind
30568	2	9019	6	NULL	NULL	0	NULL	ADR	NULL	treatment with	increases	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_10_3375_s_232	11313463	A 2.5-fold increase in p53 binding to the PIG3 promoter was observed by 4 h after ADR treatment (Fig.  2C); and although this increase in binding was accompanied by an increase in PIG3 mRNA, it was modest at 1.5-fold of the control level (Fig.  5A and B).	bind
30569	3	9019	6	NULL	NULL	0	NULL	statement 2	NULL		is accompanied by	NULL				PIG3 mRNA	NULL	increase in			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_10_3375_s_232	11313463	A 2.5-fold increase in p53 binding to the PIG3 promoter was observed by 4 h after ADR treatment (Fig.  2C); and although this increase in binding was accompanied by an increase in PIG3 mRNA, it was modest at 1.5-fold of the control level (Fig.  5A and B).	bind
38806	1	9020	5	13	NULL	NULL	NULL	p97(N-D1) hexamer	GP		bind					p47	GP		UBX domain 		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_9_1967_s_25	16601695	A 2.9  Ang  crystal structure of p97(N-D1) hexamer bound to p47(UBX) domain revealed  that p47 interacts with the p97(N) domain via a conserved loop within the UBX domain  (S3/S4) that inserts into a hydrophobic pocket between the two p97(N) subdomains  (  et al).	bind
38807	2	9020	5	13	NULL	NULL	NULL	p47	GP		interact with					p97	GP		N domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_9_1967_s_25	16601695	A 2.9  Ang  crystal structure of p97(N-D1) hexamer bound to p47(UBX) domain revealed  that p47 interacts with the p97(N) domain via a conserved loop within the UBX domain  (S3/S4) that inserts into a hydrophobic pocket between the two p97(N) subdomains  (  et al).	bind
38808	3	9020	5	13	NULL	NULL	NULL			conserved loop within	inserts into			UBX domain (S3/S4)		p97	GP		hydrophobic pocket between the two (N) subdomains		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_9_1967_s_25	16601695	A 2.9  Ang  crystal structure of p97(N-D1) hexamer bound to p47(UBX) domain revealed  that p47 interacts with the p97(N) domain via a conserved loop within the UBX domain  (S3/S4) that inserts into a hydrophobic pocket between the two p97(N) subdomains  (  et al).	bind
38809	4	9020	5	13	NULL	NULL	NULL	statement 2	Process		via					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_9_1967_s_25	16601695	A 2.9  Ang  crystal structure of p97(N-D1) hexamer bound to p47(UBX) domain revealed  that p47 interacts with the p97(N) domain via a conserved loop within the UBX domain  (S3/S4) that inserts into a hydrophobic pocket between the two p97(N) subdomains  (  et al).	bind
31169	1	9020	6	10	NULL	0	NULL	p97 (N-D1)hexamer	NULL		bind	NULL				p47	NULL		UBX domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_9_1967_s_25	16601695	A 2.9  Ang  crystal structure of p97(N-D1) hexamer bound to p47(UBX) domain revealed  that p47 interacts with the p97(N) domain via a conserved loop within the UBX domain  (S3/S4) that inserts into a hydrophobic pocket between the two p97(N) subdomains  (  et al).	bind
31170	2	9020	6	NULL	NULL	0	NULL		NULL		comprises of	NULL		UBX domain		conserved loop	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_25_9_1967_s_25	16601695	A 2.9  Ang  crystal structure of p97(N-D1) hexamer bound to p47(UBX) domain revealed  that p47 interacts with the p97(N) domain via a conserved loop within the UBX domain  (S3/S4) that inserts into a hydrophobic pocket between the two p97(N) subdomains  (  et al).	bind
31171	3	9020	6	NULL	NULL	0	NULL	statement 2	NULL		insert into	NULL				p97	NULL		hydrophobic pocket between N subdomain		NULL		0	NULL	NULL	NULL	gw70_embo_25_9_1967_s_25	16601695	A 2.9  Ang  crystal structure of p97(N-D1) hexamer bound to p47(UBX) domain revealed  that p47 interacts with the p97(N) domain via a conserved loop within the UBX domain  (S3/S4) that inserts into a hydrophobic pocket between the two p97(N) subdomains  (  et al).	bind
31172	4	9020	6	10	NULL	0	NULL	p47	NULL		interacts with	NULL				p97	NULL		N domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_9_1967_s_25	16601695	A 2.9  Ang  crystal structure of p97(N-D1) hexamer bound to p47(UBX) domain revealed  that p47 interacts with the p97(N) domain via a conserved loop within the UBX domain  (S3/S4) that inserts into a hydrophobic pocket between the two p97(N) subdomains  (  et al).	bind
47917	5	9020	6	10	NULL	0	NULL	statement 4	NULL		via	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_25_9_1967_s_25	16601695	A 2.9  Ang  crystal structure of p97(N-D1) hexamer bound to p47(UBX) domain revealed  that p47 interacts with the p97(N) domain via a conserved loop within the UBX domain  (S3/S4) that inserts into a hydrophobic pocket between the two p97(N) subdomains  (  et al).	bind
38803	2	9022	5	13	NULL	NULL	NULL	statement 1	AminoAcid		is designated as					peptide G	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_49_31179_s_18	8940117	A 20-amino acid synthetic peptide derived from the 37LRP sequence, designated peptide G, was found to bind to laminin ( 9).	bind
38804	3	9022	5	13	NULL	NULL	NULL	peptide G	AminoAcid		bind					laminin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_49_31179_s_18	8940117	A 20-amino acid synthetic peptide derived from the 37LRP sequence, designated peptide G, was found to bind to laminin ( 9).	bind
47918	1	9022	5	13	NULL	NULL	NULL	20-amino acid synthetic peptide 	AminoAcid		is derived from					37LRP sequence	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_49_31179_s_18	8940117	A 20-amino acid synthetic peptide derived from the 37LRP sequence, designated peptide G, was found to bind to laminin ( 9).	bind
30572	1	9022	6	NULL	NULL	0	NULL	peptide G	NULL		is derived from	NULL				37LRP sequence	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_49_31179_s_18	8940117	A 20-amino acid synthetic peptide derived from the 37LRP sequence, designated peptide G, was found to bind to laminin ( 9).	bind
30576	2	9022	6	NULL	NULL	0	NULL	peptide G	NULL		comprises of	NULL					NULL		20 amino acids		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_49_31179_s_18	8940117	A 20-amino acid synthetic peptide derived from the 37LRP sequence, designated peptide G, was found to bind to laminin ( 9).	bind
30577	3	9022	6	NULL	NULL	0	NULL	peptide G	NULL		bind	NULL				laminin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_49_31179_s_18	8940117	A 20-amino acid synthetic peptide derived from the 37LRP sequence, designated peptide G, was found to bind to laminin ( 9).	bind
38847	1	9024	5	13	NULL	NULL	NULL				overlaps		partially	20-bp lux box-like sequence		cepI	GP			35 region of putative promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_7_2212_s_29	11244059	A 20-bp  lux box-like sequence that partially overlaps the  35 region of the putative  cepI promoter was identified, suggesting that CepR binds to the  cepI promoter to activate  cepI expression ( 17).	bind
38848	2	9024	5	13	NULL	NULL	NULL	CepR	GP		bind					cepI	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_7_2212_s_29	11244059	A 20-bp  lux box-like sequence that partially overlaps the  35 region of the putative  cepI promoter was identified, suggesting that CepR binds to the  cepI promoter to activate  cepI expression ( 17).	bind
38849	3	9024	5	13	NULL	NULL	NULL	statement 2	Process		activates					cepI	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_7_2212_s_29	11244059	A 20-bp  lux box-like sequence that partially overlaps the  35 region of the putative  cepI promoter was identified, suggesting that CepR binds to the  cepI promoter to activate  cepI expression ( 17).	bind
38850	4	9024	5	13	NULL	NULL	NULL	statement 1	Process		suggest					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_7_2212_s_29	11244059	A 20-bp  lux box-like sequence that partially overlaps the  35 region of the putative  cepI promoter was identified, suggesting that CepR binds to the  cepI promoter to activate  cepI expression ( 17).	bind
30588	1	9024	6	NULL	NULL	0	NULL		NULL		overlaps with	NULL	partially		20-bp lux box-like sequence	CepI	NULL	putative		35 region of the promoter	NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_7_2212_s_29	11244059	A 20-bp  lux box-like sequence that partially overlaps the  35 region of the putative  cepI promoter was identified, suggesting that CepR binds to the  cepI promoter to activate  cepI expression ( 17).	bind
30589	2	9024	6	NULL	NULL	0	NULL	CepR	NULL		bind	NULL				cepI	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_7_2212_s_29	11244059	A 20-bp  lux box-like sequence that partially overlaps the  35 region of the putative  cepI promoter was identified, suggesting that CepR binds to the  cepI promoter to activate  cepI expression ( 17).	bind
30590	3	9024	6	NULL	NULL	0	NULL	statement 1	NULL		suggests	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_7_2212_s_29	11244059	A 20-bp  lux box-like sequence that partially overlaps the  35 region of the putative  cepI promoter was identified, suggesting that CepR binds to the  cepI promoter to activate  cepI expression ( 17).	bind
30591	4	9024	6	NULL	NULL	0	NULL	statement 2	NULL		activates	NULL				cepI	NULL	expression of			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_7_2212_s_29	11244059	A 20-bp  lux box-like sequence that partially overlaps the  35 region of the putative  cepI promoter was identified, suggesting that CepR binds to the  cepI promoter to activate  cepI expression ( 17).	bind
38851	1	9026	5	13	NULL	NULL	NULL	Ab C-597	GP		bind					PROT proteins	GP	native			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_26_15755_s_90	7797577	A 20-fold excess of peptide  efficiently blocked binding of Ab C-597 to native PROT proteins.	bind
30596	1	9026	6	NULL	NULL	0	NULL	Ab C-597	NULL		bind	NULL				PROT proteins	NULL	native			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_26_15755_s_90	7797577	A 20-fold excess of peptide  efficiently blocked binding of Ab C-597 to native PROT proteins.	bind
38852	1	9027	5	13	NULL	NULL	NULL	20-residue peptide	AminoAcid		encode					Cav ce	GP		predicted G protein binding region		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2437_s_15	8999956	A 20-residue peptide encoding the predicted G protein binding region of Cav ce possesses "`GDP dissociation inhibitor-like activity"` with the same potency as described earlier for mammalian caveolin-1.	bind
38853	2	9027	5	13	NULL	NULL	NULL	statement 1	AminoAcid		possesses					GDP dissociation inhibitor-like activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2437_s_15	8999956	A 20-residue peptide encoding the predicted G protein binding region of Cav ce possesses "`GDP dissociation inhibitor-like activity"` with the same potency as described earlier for mammalian caveolin-1.	bind
38854	3	9027	5	13	NULL	NULL	NULL	caveolin-1	GP	mammalian	possess					GDP dissociation inhibitor-like activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2437_s_15	8999956	A 20-residue peptide encoding the predicted G protein binding region of Cav ce possesses "`GDP dissociation inhibitor-like activity"` with the same potency as described earlier for mammalian caveolin-1.	bind
57756	4	9027	5	13	NULL	NULL	NULL	statement 2	Process		same potency as					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2437_s_15	8999956	A 20-residue peptide encoding the predicted G protein binding region of Cav ce possesses "`GDP dissociation inhibitor-like activity"` with the same potency as described earlier for mammalian caveolin-1.	bind
31173	2	9027	6	10	NULL	0	NULL	statement 1			possesses					GDP dissociation inhibitor-like activity					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2437_s_15	8999956	A 20-residue peptide encoding the predicted G protein binding region of Cav ce possesses "`GDP dissociation inhibitor-like activity"` with the same potency as described earlier for mammalian caveolin-1.	bind
31174	3	9027	6	10	NULL	0	NULL	Caveolin-1		mammalian	possesses					GDP dissociation inhibitor-like activity					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2437_s_15	8999956	A 20-residue peptide encoding the predicted G protein binding region of Cav ce possesses "`GDP dissociation inhibitor-like activity"` with the same potency as described earlier for mammalian caveolin-1.	bind
31175	4	9027	6	10	NULL	0	NULL	statement 2			same potency as					statement 3					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2437_s_15	8999956	A 20-residue peptide encoding the predicted G protein binding region of Cav ce possesses "`GDP dissociation inhibitor-like activity"` with the same potency as described earlier for mammalian caveolin-1.	bind
57757	1	9027	6	10	NULL	0	NULL	20-residue peptide			encode					Cav ce			 predicted G protein binding region		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_4_2437_s_15	8999956	A 20-residue peptide encoding the predicted G protein binding region of Cav ce possesses "`GDP dissociation inhibitor-like activity"` with the same potency as described earlier for mammalian caveolin-1.	bind
38855	1	9028	5	13	NULL	NULL	NULL	CPD	GP		bind			20-residue region within the cytoplasmic tail		PP2A	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-cell-sci_114_pt-2_11148133_s_3	11148133	A 20-residue region within the cytoplasmic  tail of CPD binds protein phosphatase 2A (PP2A).	bind
38856	2	9028	5	13	NULL	NULL	NULL	PP2A	GP		is					protein phosphatase 2A	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-cell-sci_114_pt-2_11148133_s_3	11148133	A 20-residue region within the cytoplasmic  tail of CPD binds protein phosphatase 2A (PP2A).	bind
30601	1	9028	6	NULL	NULL	0	NULL	CPD	NULL		bind	NULL		20-residue region within the cytoplasmic tail		PP2A	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-cell-sci_114_pt-2_11148133_s_3	11148133	A 20-residue region within the cytoplasmic  tail of CPD binds protein phosphatase 2A (PP2A).	bind
30602	2	9028	6	NULL	NULL	0	NULL	PP2A	NULL		is	NULL				protein phosphatase 2A	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-cell-sci_114_pt-2_11148133_s_3	11148133	A 20-residue region within the cytoplasmic  tail of CPD binds protein phosphatase 2A (PP2A).	bind
38857	1	9029	5	13	NULL	NULL	NULL	RBD-Ig of TOR2 variants	GP	purified	bind					Sigma I-2136	GP	immobilized			NULL		NULL	NULL	NULL	NULL	gw70_embo_24_8_1634_s_252	15791205	A 200 nM portion of purified RBD-Ig of TOR2 variants was bound to an anti-human  antibody (Sigma I-2136) immobilized on a CM5 sensor chip.	bind
38858	2	9029	5	13	NULL	NULL	NULL	Sigma I-2136	GP		is a type of					anti-human antibody	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_8_1634_s_252	15791205	A 200 nM portion of purified RBD-Ig of TOR2 variants was bound to an anti-human  antibody (Sigma I-2136) immobilized on a CM5 sensor chip.	bind
30603	1	9029	6	10	NULL	0	NULL	Sigma I-2136	NULL		is a type of	NULL				anti-human antibody	NULL				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_8_1634_s_252	15791205	A 200 nM portion of purified RBD-Ig of TOR2 variants was bound to an anti-human  antibody (Sigma I-2136) immobilized on a CM5 sensor chip.	bind
30605	2	9029	6	10	NULL	0	NULL	RBD-Ig of TOR2 variants	NULL	purified	bind	NULL				Sigma I-2136	NULL				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_8_1634_s_252	15791205	A 200 nM portion of purified RBD-Ig of TOR2 variants was bound to an anti-human  antibody (Sigma I-2136) immobilized on a CM5 sensor chip.	bind
38859	1	9030	5	13	NULL	NULL	NULL	osk	GP		bind					Hrb27C	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_131_9_1949_s_155	15056611	A 200-fold excess  grk or  osk is able to compete binding of Hrb27C (arrow) from  osk, while excess  nos is not.	bind
38862	2	9030	5	13	NULL	NULL	NULL	grk	GP	excess	bind					Hrb27C	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_131_9_1949_s_155	15056611	A 200-fold excess  grk or  osk is able to compete binding of Hrb27C (arrow) from  osk, while excess  nos is not.	bind
38863	3	9030	5	13	NULL	NULL	NULL	statement 2	Process		competes with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_131_9_1949_s_155	15056611	A 200-fold excess  grk or  osk is able to compete binding of Hrb27C (arrow) from  osk, while excess  nos is not.	bind
57758	4	9030	5	13	NULL	NULL	NULL	nos	GP	excess of	does not compete with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_131_9_1949_s_155	15056611	A 200-fold excess  grk or  osk is able to compete binding of Hrb27C (arrow) from  osk, while excess  nos is not.	bind
57759	5	9030	5	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_131_9_1949_s_155	15056611	A 200-fold excess  grk or  osk is able to compete binding of Hrb27C (arrow) from  osk, while excess  nos is not.	bind
30607	1	9030	6	NULL	NULL	0	NULL	Hrb27C	NULL		bind	NULL				osk	NULL				NULL		0	NULL	NULL	NULL	gw70_development_131_9_1949_s_155	15056611	A 200-fold excess  grk or  osk is able to compete binding of Hrb27C (arrow) from  osk, while excess  nos is not.	bind
30608	2	9030	6	NULL	NULL	0	NULL	grk	NULL	excess of	bind	NULL				osk	NULL				NULL		0	NULL	NULL	NULL	gw70_development_131_9_1949_s_155	15056611	A 200-fold excess  grk or  osk is able to compete binding of Hrb27C (arrow) from  osk, while excess  nos is not.	bind
30609	3	9030	6	NULL	NULL	0	NULL	statement 1	NULL		competes	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_development_131_9_1949_s_155	15056611	A 200-fold excess  grk or  osk is able to compete binding of Hrb27C (arrow) from  osk, while excess  nos is not.	bind
30612	5	9030	6	10	NULL	0	NULL	statement 1			is an alternative to					statement 2					NULL		NULL	NULL	NULL	NULL	gw70_development_131_9_1949_s_155	15056611	A 200-fold excess  grk or  osk is able to compete binding of Hrb27C (arrow) from  osk, while excess  nos is not.	bind
30613	4	9030	6	10	NULL	0	NULL	nos		excess of	does not compete with					statement 1					NULL		NULL	NULL	NULL	NULL	gw70_development_131_9_1949_s_155	15056611	A 200-fold excess  grk or  osk is able to compete binding of Hrb27C (arrow) from  osk, while excess  nos is not.	bind
42524	1	9031	5	13	NULL	NULL	NULL	HNF-3beta complex	GP		bind					HNF-3 consensus probe	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_34_26637_s_181	10859308	A 200-fold excess of nonradioactive site 1 oligonucleotide competes well for binding of the HNF-3 consensus probe for the upper HNF-3beta complex ( lane 3).	bind
30614	1	9031	6	NULL	NULL	0	NULL	HNF-3beta complex	NULL		bind	NULL				HNF-3 consensus probe	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_34_26637_s_181	10859308	A 200-fold excess of nonradioactive site 1 oligonucleotide competes well for binding of the HNF-3 consensus probe for the upper HNF-3beta complex ( lane 3).	bind
38864	1	9032	5	13	NULL	NULL	NULL	consensus Sp1 oligonucleotide probe	NucleicAcid		bind					Sp1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_47_43713_s_173	11559712	A 200-fold molar excess of a consensus Sp1 oligonucleotide probe (which binds Sp1 and Sp3) competed for the binding of NF-1 and NF-3 but not the other complexes.	bind
38865	2	9032	5	13	NULL	NULL	NULL	consensus Sp1 oligonucleotide probe	NucleicAcid		bind					Sp3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_47_43713_s_173	11559712	A 200-fold molar excess of a consensus Sp1 oligonucleotide probe (which binds Sp1 and Sp3) competed for the binding of NF-1 and NF-3 but not the other complexes.	bind
38866	3	9032	5	13	NULL	NULL	NULL	consensus Sp1 oligonucleotide probe	NucleicAcid		bind					NF-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_47_43713_s_173	11559712	A 200-fold molar excess of a consensus Sp1 oligonucleotide probe (which binds Sp1 and Sp3) competed for the binding of NF-1 and NF-3 but not the other complexes.	bind
38867	4	9032	5	13	NULL	NULL	NULL	consensus Sp1 oligonucleotide probe	NucleicAcid		bind					NF-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_47_43713_s_173	11559712	A 200-fold molar excess of a consensus Sp1 oligonucleotide probe (which binds Sp1 and Sp3) competed for the binding of NF-1 and NF-3 but not the other complexes.	bind
38868	5	9032	5	13	NULL	NULL	NULL	statement 3	Process		competes with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_47_43713_s_173	11559712	A 200-fold molar excess of a consensus Sp1 oligonucleotide probe (which binds Sp1 and Sp3) competed for the binding of NF-1 and NF-3 but not the other complexes.	bind
30617	1	9032	6	NULL	NULL	0	NULL	Sp1 oligonucleotide probe	NULL		bind	NULL				Sp1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_47_43713_s_173	11559712	A 200-fold molar excess of a consensus Sp1 oligonucleotide probe (which binds Sp1 and Sp3) competed for the binding of NF-1 and NF-3 but not the other complexes.	bind
30618	2	9032	6	NULL	NULL	0	NULL	Sp1 oligonucleotide probe	NULL		bind	NULL				Sp3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_47_43713_s_173	11559712	A 200-fold molar excess of a consensus Sp1 oligonucleotide probe (which binds Sp1 and Sp3) competed for the binding of NF-1 and NF-3 but not the other complexes.	bind
30619	3	9032	6	10	NULL	0	NULL	 Sp1 oligonucleotide probe	NULL		bind	NULL				NF-1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_47_43713_s_173	11559712	A 200-fold molar excess of a consensus Sp1 oligonucleotide probe (which binds Sp1 and Sp3) competed for the binding of NF-1 and NF-3 but not the other complexes.	bind
30621	4	9032	6	NULL	NULL	0	NULL	Sp1 oligonucleotide probe	NULL	excess of	bind	NULL				NF-3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_47_43713_s_173	11559712	A 200-fold molar excess of a consensus Sp1 oligonucleotide probe (which binds Sp1 and Sp3) competed for the binding of NF-1 and NF-3 but not the other complexes.	bind
30622	5	9032	6	NULL	NULL	0	NULL	statement 4	NULL		competes	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_47_43713_s_173	11559712	A 200-fold molar excess of a consensus Sp1 oligonucleotide probe (which binds Sp1 and Sp3) competed for the binding of NF-1 and NF-3 but not the other complexes.	bind
38869	1	9033	5	13	NULL	NULL	NULL	isl-1	GP		bind					Ga probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_21_12646_s_62	7759514	A 200-fold molar excess of unlabeled Ga markedly  diminished the binding of  isl-1  to the Ga probe  ( Fig. 1).	bind
38871	2	9033	5	13	NULL	NULL	NULL	Ga	GP	excess;;unlabeled	diminished		markedly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_21_12646_s_62	7759514	A 200-fold molar excess of unlabeled Ga markedly  diminished the binding of  isl-1  to the Ga probe  ( Fig. 1).	bind
30623	1	9033	6	NULL	NULL	0	NULL	isl-1	NULL		bind	NULL				Ga probe	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_21_12646_s_62	7759514	A 200-fold molar excess of unlabeled Ga markedly  diminished the binding of  isl-1  to the Ga probe  ( Fig. 1).	bind
30624	2	9033	6	NULL	NULL	0	NULL	Ga	NULL	excess of;; unlabeled	diminishes	NULL	markedly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_21_12646_s_62	7759514	A 200-fold molar excess of unlabeled Ga markedly  diminished the binding of  isl-1  to the Ga probe  ( Fig. 1).	bind
38872	1	9034	5	13	NULL	NULL	NULL	21 kDa surface protein	GP	Mycobacterium leprae	bind					peripheral nerve laminin-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_3_511_s_521	11081637	A 21 kDa surface protein of  Mycobacterium leprae binds peripheral nerve laminin-2 and mediates Schwann cell invasion.	bind
38873	2	9034	5	13	NULL	NULL	NULL	statement 1	Process		mediate					Schwann cell 	Cell	invasion of			NULL		NULL	NULL	NULL	NULL	gw60_cell_103_3_511_s_521	11081637	A 21 kDa surface protein of  Mycobacterium leprae binds peripheral nerve laminin-2 and mediates Schwann cell invasion.	bind
30627	1	9034	6	NULL	NULL	0	NULL	21 kDa surface protein	NULL	Mycobacterium leprae	bind	NULL				peripheral nerve laminin-2	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_103_3_511_s_521	11081637	A 21 kDa surface protein of  Mycobacterium leprae binds peripheral nerve laminin-2 and mediates Schwann cell invasion.	bind
30629	2	9034	6	NULL	NULL	0	NULL	statement 1	NULL		mediates	NULL				Schwann cell 	NULL	invasion of 			NULL		0	NULL	NULL	NULL	gw60_cell_103_3_511_s_521	11081637	A 21 kDa surface protein of  Mycobacterium leprae binds peripheral nerve laminin-2 and mediates Schwann cell invasion.	bind
38875	1	9038	5	13	NULL	NULL	NULL	Ht31	GP	full-length	bind					RII	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_38_23637_s_31	9295304	A 22-residue peptide mimicking the RII binding site of Ht31 has been synthesized which inhibits the binding of full-length Ht31 binding to RII ( 17).	bind
38876	2	9038	5	13	NULL	NULL	NULL	22-residue peptide	GP		mimick					Ht31	GP		RII binding site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_38_23637_s_31	9295304	A 22-residue peptide mimicking the RII binding site of Ht31 has been synthesized which inhibits the binding of full-length Ht31 binding to RII ( 17).	bind
38877	3	9038	5	13	NULL	NULL	NULL	statement 2	Process	synthesized	inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_38_23637_s_31	9295304	A 22-residue peptide mimicking the RII binding site of Ht31 has been synthesized which inhibits the binding of full-length Ht31 binding to RII ( 17).	bind
30654	1	9038	6	NULL	NULL	0	NULL	Ht31	NULL		bind	NULL				RII	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_38_23637_s_31	9295304	A 22-residue peptide mimicking the RII binding site of Ht31 has been synthesized which inhibits the binding of full-length Ht31 binding to RII ( 17).	bind
30655	3	9038	6	10	NULL	0	NULL	statement 2		synthesized	inhibits					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_38_23637_s_31	9295304	A 22-residue peptide mimicking the RII binding site of Ht31 has been synthesized which inhibits the binding of full-length Ht31 binding to RII ( 17).	bind
57760	2	9038	6	10	NULL	0	NULL	22-residue peptide			mimicks					Ht31			RII binding site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_38_23637_s_31	9295304	A 22-residue peptide mimicking the RII binding site of Ht31 has been synthesized which inhibits the binding of full-length Ht31 binding to RII ( 17).	bind
38878	1	9039	5	13	NULL	NULL	NULL	s-Sec1	GP		bind					s-syntaxin	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jneurosci_18_8_2923_s_6	9526009	A 24 amino acid peptide fragment of s-Sec1, which inhibited the binding of s-Sec1 to s-syntaxin   in vitro, completely blocked release, suggesting an essential function of the s-Sec1/s-syntaxin interaction in transmitter release.	bind
38879	2	9039	5	13	NULL	NULL	NULL	s-Sec1	GP		inhibit			24 amino acid peptide fragment of 		statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jneurosci_18_8_2923_s_6	9526009	A 24 amino acid peptide fragment of s-Sec1, which inhibited the binding of s-Sec1 to s-syntaxin   in vitro, completely blocked release, suggesting an essential function of the s-Sec1/s-syntaxin interaction in transmitter release.	bind
38880	4	9039	5	13	NULL	NULL	NULL	statement 2	Process		block		completely			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_18_8_2923_s_6	9526009	A 24 amino acid peptide fragment of s-Sec1, which inhibited the binding of s-Sec1 to s-syntaxin   in vitro, completely blocked release, suggesting an essential function of the s-Sec1/s-syntaxin interaction in transmitter release.	bind
38881	3	9039	5	13	NULL	NULL	NULL	statement 1	Process		function in					transmitter 	Chemical	release of			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_18_8_2923_s_6	9526009	A 24 amino acid peptide fragment of s-Sec1, which inhibited the binding of s-Sec1 to s-syntaxin   in vitro, completely blocked release, suggesting an essential function of the s-Sec1/s-syntaxin interaction in transmitter release.	bind
30656	1	9039	6	NULL	NULL	0	NULL	s-Sec1	NULL		bind	NULL				s-syntaxin	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_jneurosci_18_8_2923_s_6	9526009	A 24 amino acid peptide fragment of s-Sec1, which inhibited the binding of s-Sec1 to s-syntaxin   in vitro, completely blocked release, suggesting an essential function of the s-Sec1/s-syntaxin interaction in transmitter release.	bind
30657	2	9039	6	10	NULL	0	NULL	s-Sec1			inhibits			24 amino acid peptide fragment of 		statement 1					NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jneurosci_18_8_2923_s_6	9526009	A 24 amino acid peptide fragment of s-Sec1, which inhibited the binding of s-Sec1 to s-syntaxin   in vitro, completely blocked release, suggesting an essential function of the s-Sec1/s-syntaxin interaction in transmitter release.	bind
30658	3	9039	6	NULL	NULL	0	NULL	statement 1	NULL		plays a role in	NULL				transmitter	NULL	release of 			NULL		0	NULL	NULL	NULL	gw60_jneurosci_18_8_2923_s_6	9526009	A 24 amino acid peptide fragment of s-Sec1, which inhibited the binding of s-Sec1 to s-syntaxin   in vitro, completely blocked release, suggesting an essential function of the s-Sec1/s-syntaxin interaction in transmitter release.	bind
47976	4	9039	6	10	NULL	0	NULL	statement 2	NULL		block	NULL	completely			statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_18_8_2923_s_6	9526009	A 24 amino acid peptide fragment of s-Sec1, which inhibited the binding of s-Sec1 to s-syntaxin   in vitro, completely blocked release, suggesting an essential function of the s-Sec1/s-syntaxin interaction in transmitter release.	bind
38883	1	9040	5	13	NULL	NULL	NULL	 Tat-p21 fusion peptide	GP		encompass					nuclear localization signal	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3364_s_317	15798220	A 24-amino-acid Tat-p21 fusion peptide encompassing the nuclear localization signal  and the PCNA-binding region of p21 blocks p21 phosphorylation and results in cell  death.	bind
38884	4	9040	5	13	NULL	NULL	NULL	statement 3	Process		results in					cell death	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3364_s_317	15798220	A 24-amino-acid Tat-p21 fusion peptide encompassing the nuclear localization signal  and the PCNA-binding region of p21 blocks p21 phosphorylation and results in cell  death.	bind
47977	2	9040	5	13	NULL	NULL	NULL	Tat-p21 fusion peptide	GP		encompass					p21	GP		PCNA-binding region 		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3364_s_317	15798220	A 24-amino-acid Tat-p21 fusion peptide encompassing the nuclear localization signal  and the PCNA-binding region of p21 blocks p21 phosphorylation and results in cell  death.	bind
47978	3	9040	5	13	NULL	NULL	NULL	Tat-p21 fusion peptide	GP		blocks					p21	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3364_s_317	15798220	A 24-amino-acid Tat-p21 fusion peptide encompassing the nuclear localization signal  and the PCNA-binding region of p21 blocks p21 phosphorylation and results in cell  death.	bind
47979	5	9040	5	13	NULL	NULL	NULL	Tat-p21 fusion peptide	GP		contains					24-amino-acid	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_3364_s_317	15798220	A 24-amino-acid Tat-p21 fusion peptide encompassing the nuclear localization signal  and the PCNA-binding region of p21 blocks p21 phosphorylation and results in cell  death.	bind
31176	1	9040	6	NULL	NULL	0	NULL	Tat-p21 fusion peptide	NULL		encompasses	NULL				nuclear localization signal	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_8_3364_s_317	15798220	A 24-amino-acid Tat-p21 fusion peptide encompassing the nuclear localization signal  and the PCNA-binding region of p21 blocks p21 phosphorylation and results in cell  death.	bind
31177	2	9040	6	NULL	NULL	0	NULL	Tat-p21 fusion peptide	NULL		comprises	NULL				p21	NULL		PCNA binding region		NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_8_3364_s_317	15798220	A 24-amino-acid Tat-p21 fusion peptide encompassing the nuclear localization signal  and the PCNA-binding region of p21 blocks p21 phosphorylation and results in cell  death.	bind
31178	3	9040	6	NULL	NULL	0	NULL	Tat-p21 fusion peptide	NULL		blocks	NULL				p21	NULL	phosphorylation of 			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_8_3364_s_317	15798220	A 24-amino-acid Tat-p21 fusion peptide encompassing the nuclear localization signal  and the PCNA-binding region of p21 blocks p21 phosphorylation and results in cell  death.	bind
31179	4	9040	6	NULL	NULL	0	NULL	statement 3	NULL		leads to	NULL				cell death	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_8_3364_s_317	15798220	A 24-amino-acid Tat-p21 fusion peptide encompassing the nuclear localization signal  and the PCNA-binding region of p21 blocks p21 phosphorylation and results in cell  death.	bind
47980	5	9040	6	10	NULL	0	NULL	Tat-p21 fusion peptide	NULL		contains	NULL				24-amino-acid	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_8_3364_s_317	15798220	A 24-amino-acid Tat-p21 fusion peptide encompassing the nuclear localization signal  and the PCNA-binding region of p21 blocks p21 phosphorylation and results in cell  death.	bind
38885	1	9042	5	13	NULL	NULL	NULL	ORF3 protein	GP		bind			25-amino acid region		ORF2 protein	GP	full length			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_25_22759_s_158	11934888	A 25-Amino Acid Region of the ORF3 Protein Binds to the Full-length ORF2 Protein-- To characterize the domains involved in the ORF2-ORF3 interaction, an array of deletion mutations were constructed for both ORF2 and ORF3 and were cloned into the yeast two-hybrid AD and BD vectors as described in Table  I. Combinations of full-length fusion constructs and deletion mutants of each fusion construct were tested for  in vivo protein-protein interactions as shown in Fig.  5.	bind
30660	1	9042	6	NULL	NULL	0	NULL	ORF3 protein	NULL		bind	NULL		25-Amino Acid Region		ORF2 protein	NULL	full length			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_25_22759_s_158	11934888	A 25-Amino Acid Region of the ORF3 Protein Binds to the Full-length ORF2 Protein-- To characterize the domains involved in the ORF2-ORF3 interaction, an array of deletion mutations were constructed for both ORF2 and ORF3 and were cloned into the yeast two-hybrid AD and BD vectors as described in Table  I. Combinations of full-length fusion constructs and deletion mutants of each fusion construct were tested for  in vivo protein-protein interactions as shown in Fig.  5.	bind
38886	1	9043	5	13	NULL	NULL	NULL	Cyp2b10 gene	GP		bind				25-bp DNA fragment	nuclear protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_16_9746_s_232	8621653	A 25-bp DNA fragment at -1.2 kilobase pairs of  Cyp2b10  gene is 80%  similar to a portion of the 163-bp  sequence, and an overlapping segment (-1228/-1195 bp) can  bind nuclear protein(s).	bind
47981	1	9043	6	10	NULL	0	NULL	Cyp2b10 gene	NULL		bind	NULL			25-bp DNA fragment	nuclear proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_16_9746_s_232	8621653	A 25-bp DNA fragment at -1.2 kilobase pairs of  Cyp2b10  gene is 80%  similar to a portion of the 163-bp  sequence, and an overlapping segment (-1228/-1195 bp) can  bind nuclear protein(s).	bind
38888	1	9045	5	13	NULL	NULL	NULL				bind			26 S protease subunit		ubiquitin conjugates	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_140_3_499_s_377	9456312	A 26 S protease  subunit that binds ubiquitin conjugates.	bind
30661	1	9045	6	10	NULL	0	NULL				bind			26 S protease subunit		ubiquitin conjugates					NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_140_3_499_s_377	9456312	A 26 S protease  subunit that binds ubiquitin conjugates.	bind
38889	1	9048	5	13	NULL	NULL	NULL	S5a	GP		is a type of					26 S proteasome subunit	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_51_32538_s_231	8955078	A 26 S proteasome subunit (S5a) that binds Ub-conjugate substrates has already been identified and its cDNA has been cloned and expressed ( 61,  62).	bind
38890	2	9048	5	13	NULL	NULL	NULL	S5a	GP		bind					Ub-conjugate substrates	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_51_32538_s_231	8955078	A 26 S proteasome subunit (S5a) that binds Ub-conjugate substrates has already been identified and its cDNA has been cloned and expressed ( 61,  62).	bind
30662	1	9048	6	10	NULL	0	NULL	S5a	NULL		bind	NULL				Ub-conjugate substrate	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_51_32538_s_231	8955078	A 26 S proteasome subunit (S5a) that binds Ub-conjugate substrates has already been identified and its cDNA has been cloned and expressed ( 61,  62).	bind
30663	2	9048	6	10	NULL	0	NULL	S5a	NULL		is a type of	NULL				 26 S proteasome subunit	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_51_32538_s_231	8955078	A 26 S proteasome subunit (S5a) that binds Ub-conjugate substrates has already been identified and its cDNA has been cloned and expressed ( 61,  62).	bind
38891	1	9050	5	13	NULL	NULL	NULL	UBA molecules	GP		bind					Ub2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_8_7055_s_111	14645257	A 2:1 model, in addition, allows up to two UBA molecules bound to Ub2, one per Ub unit.	bind
30664	1	9050	6	NULL	NULL	0	NULL	UBA molecule	NULL		bind	NULL				Ub2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_7055_s_111	14645257	A 2:1 model, in addition, allows up to two UBA molecules bound to Ub2, one per Ub unit.	bind
38892	1	9051	5	13	NULL	NULL	NULL	zipper protein	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_15_9075_s_239	8621557	A 2:1 molar ratio of zipper  protein to actin appears to be maximally effective and is sufficient to  saturate binding of zipper protein to actin.	bind
30665	1	9051	6	NULL	NULL	0	NULL	zipper protein	NULL		bind	NULL				actin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_15_9075_s_239	8621557	A 2:1 molar ratio of zipper  protein to actin appears to be maximally effective and is sufficient to  saturate binding of zipper protein to actin.	bind
38893	1	9053	5	13	NULL	NULL	NULL	GTP	Chemical		bind					eIF-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_18_2396_s_320	9308967	A 3-bp codon/anticodon interaction occurs, which signals the eIF-5-dependent hydrolysis of GTP bound to eIF-2.	bind
38894	2	9053	5	13	NULL	NULL	NULL	statement 1	Process	hydrolysis of	is dependent on					eIF-5	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_18_2396_s_320	9308967	A 3-bp codon/anticodon interaction occurs, which signals the eIF-5-dependent hydrolysis of GTP bound to eIF-2.	bind
38895	4	9053	5	13	NULL	NULL	NULL	statement 3	Process		signals					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_18_2396_s_320	9308967	A 3-bp codon/anticodon interaction occurs, which signals the eIF-5-dependent hydrolysis of GTP bound to eIF-2.	bind
47982	3	9053	5	13	NULL	NULL	NULL	3-bp codon	NucleicAcid		interacts with					anticodon	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_18_2396_s_320	9308967	A 3-bp codon/anticodon interaction occurs, which signals the eIF-5-dependent hydrolysis of GTP bound to eIF-2.	bind
30848	1	9053	6	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				eIF-2	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_11_18_2396_s_320	9308967	A 3-bp codon/anticodon interaction occurs, which signals the eIF-5-dependent hydrolysis of GTP bound to eIF-2.	bind
30849	2	9053	6	NULL	NULL	0	NULL	statement 1	NULL	hydrolysis of	is dependent on	NULL				eIF-5	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_11_18_2396_s_320	9308967	A 3-bp codon/anticodon interaction occurs, which signals the eIF-5-dependent hydrolysis of GTP bound to eIF-2.	bind
30850	3	9053	6	NULL	NULL	0	NULL	3-bp codon	NULL		interacts with	NULL				anticodon	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_11_18_2396_s_320	9308967	A 3-bp codon/anticodon interaction occurs, which signals the eIF-5-dependent hydrolysis of GTP bound to eIF-2.	bind
30851	4	9053	6	NULL	NULL	0	NULL	statement 3	NULL		signals	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_11_18_2396_s_320	9308967	A 3-bp codon/anticodon interaction occurs, which signals the eIF-5-dependent hydrolysis of GTP bound to eIF-2.	bind
38896	1	9054	5	13	NULL	NULL	NULL	HisP	GP		is a type of					nucleotide-binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_5_554_s_5	11909819	A 3-D structure model of the region containing the second nucleotide-binding domain (NBD2) of SUR and C42 was developed based on the structure of HisP, a nucleotide-binding protein forming the bacterial Histidine transporter complex.	bind
38898	2	9054	5	13	NULL	NULL	NULL	HisP	GP		forms					Histidine transporter complex	GP	bacterial			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_5_554_s_5	11909819	A 3-D structure model of the region containing the second nucleotide-binding domain (NBD2) of SUR and C42 was developed based on the structure of HisP, a nucleotide-binding protein forming the bacterial Histidine transporter complex.	bind
47983	3	9054	5	13	NULL	NULL	NULL	NBD2	GP		is					nucleotide-binding domain	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_5_554_s_5	11909819	A 3-D structure model of the region containing the second nucleotide-binding domain (NBD2) of SUR and C42 was developed based on the structure of HisP, a nucleotide-binding protein forming the bacterial Histidine transporter complex.	bind
30852	1	9054	6	NULL	NULL	0	NULL	HisP	NULL		is a type of	NULL				nucleotide-binding protein	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_90_5_554_s_5	11909819	A 3-D structure model of the region containing the second nucleotide-binding domain (NBD2) of SUR and C42 was developed based on the structure of HisP, a nucleotide-binding protein forming the bacterial Histidine transporter complex.	bind
30853	2	9054	6	10	NULL	0	NULL	HisP			forms					 Histidine transporter complex		bacterial			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_5_554_s_5	11909819	A 3-D structure model of the region containing the second nucleotide-binding domain (NBD2) of SUR and C42 was developed based on the structure of HisP, a nucleotide-binding protein forming the bacterial Histidine transporter complex.	bind
30854	3	9054	6	10	NULL	0	NULL	NBD2	NULL		is	NULL				nucleotide-binding domain	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_5_554_s_5	11909819	A 3-D structure model of the region containing the second nucleotide-binding domain (NBD2) of SUR and C42 was developed based on the structure of HisP, a nucleotide-binding protein forming the bacterial Histidine transporter complex.	bind
38900	1	9056	5	13	NULL	NULL	NULL	MTSEA	Chemical		inhibit		strongly					binding properties of ;;mutant	A104C		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_49_51415_s_102	15452107	A 3-min treatment with 0.5 mM MTSEA ( Fig. 3 A) strongly inhibited the binding properties of mutants A104C(3.28) and L112C(3.36), whereas it had only a minor effect on the binding properties of the other mutant receptors.	bind
38901	2	9056	5	13	NULL	NULL	NULL	MTSEA	Chemical		inhibit		strongly					binding properties of;;mutant	L112C		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_49_51415_s_102	15452107	A 3-min treatment with 0.5 mM MTSEA ( Fig. 3 A) strongly inhibited the binding properties of mutants A104C(3.28) and L112C(3.36), whereas it had only a minor effect on the binding properties of the other mutant receptors.	bind
30855	1	9056	6	NULL	NULL	0	NULL	MTSEA	NULL		inhibits	NULL	strongly				NULL	binding properties of;; mutant	A104C		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_49_51415_s_102	15452107	A 3-min treatment with 0.5 mM MTSEA ( Fig. 3 A) strongly inhibited the binding properties of mutants A104C(3.28) and L112C(3.36), whereas it had only a minor effect on the binding properties of the other mutant receptors.	bind
30856	2	9056	6	NULL	NULL	0	NULL	MTSEA	NULL		inhibits	NULL	strongly				NULL	binding properties of;; mutant	L112C		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_49_51415_s_102	15452107	A 3-min treatment with 0.5 mM MTSEA ( Fig. 3 A) strongly inhibited the binding properties of mutants A104C(3.28) and L112C(3.36), whereas it had only a minor effect on the binding properties of the other mutant receptors.	bind
38902	1	9058	5	13	NULL	NULL	NULL	alpha1(V) chain	GP		bind			heparin-binding fragment 		heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29377_s_15	10862775	A 30-kDa heparin-binding fragment of the alpha1(V) chain has been isolated and was shown to bind heparin with the same affinity as the complete parental chain ( 12).	bind
38903	2	9058	5	13	NULL	NULL	NULL	alpha1(V) chain	GP	complete parental chain	bind					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29377_s_15	10862775	A 30-kDa heparin-binding fragment of the alpha1(V) chain has been isolated and was shown to bind heparin with the same affinity as the complete parental chain ( 12).	bind
38904	3	9058	5	13	NULL	NULL	NULL	statement 1	Process		same affinity as					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29377_s_15	10862775	A 30-kDa heparin-binding fragment of the alpha1(V) chain has been isolated and was shown to bind heparin with the same affinity as the complete parental chain ( 12).	bind
30858	1	9058	6	NULL	NULL	0	NULL	alpha1(V) chain	NULL		bind	NULL		heparin binding fragment		heparin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29377_s_15	10862775	A 30-kDa heparin-binding fragment of the alpha1(V) chain has been isolated and was shown to bind heparin with the same affinity as the complete parental chain ( 12).	bind
30859	2	9058	6	10	NULL	0	NULL	alpha1(V) chain	NULL	complete	bind	NULL				heparin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29377_s_15	10862775	A 30-kDa heparin-binding fragment of the alpha1(V) chain has been isolated and was shown to bind heparin with the same affinity as the complete parental chain ( 12).	bind
30860	3	9058	6	NULL	NULL	0	NULL	statement 1	NULL	affinity of	is same as	NULL				statement 2	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29377_s_15	10862775	A 30-kDa heparin-binding fragment of the alpha1(V) chain has been isolated and was shown to bind heparin with the same affinity as the complete parental chain ( 12).	bind
38905	1	9059	5	13	NULL	NULL	NULL	CBP/p300	GP		bind					CREB	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_8_3697_s_32	9108040	A 300-kDa protein (CBP/p300) which binds to the cAMP response element-binding protein (CREB) functions as a coactivator of CREB-mediated signaling pathways.	bind
38906	2	9059	5	13	NULL	NULL	NULL	CREB	GP		is					cAMP response element-binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_8_3697_s_32	9108040	A 300-kDa protein (CBP/p300) which binds to the cAMP response element-binding protein (CREB) functions as a coactivator of CREB-mediated signaling pathways.	bind
38907	3	9059	5	13	NULL	NULL	NULL	CREB	GP		function as					coactivator	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_8_3697_s_32	9108040	A 300-kDa protein (CBP/p300) which binds to the cAMP response element-binding protein (CREB) functions as a coactivator of CREB-mediated signaling pathways.	bind
47984	4	9059	5	13	NULL	NULL	NULL	CREB	GP		mediates					signaling pathways	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_8_3697_s_32	9108040	A 300-kDa protein (CBP/p300) which binds to the cAMP response element-binding protein (CREB) functions as a coactivator of CREB-mediated signaling pathways.	bind
47985	5	9059	5	13	NULL	NULL	NULL	statement 3	Process		occurs in					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_8_3697_s_32	9108040	A 300-kDa protein (CBP/p300) which binds to the cAMP response element-binding protein (CREB) functions as a coactivator of CREB-mediated signaling pathways.	bind
47986	6	9059	5	13	NULL	NULL	NULL	CBP/p300	GP		is a type of					300-kDa protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_8_3697_s_32	9108040	A 300-kDa protein (CBP/p300) which binds to the cAMP response element-binding protein (CREB) functions as a coactivator of CREB-mediated signaling pathways.	bind
30861	1	9059	6	NULL	NULL	0	NULL	CREB	NULL		is	NULL				cAMP response element-binding protein	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_94_8_3697_s_32	9108040	A 300-kDa protein (CBP/p300) which binds to the cAMP response element-binding protein (CREB) functions as a coactivator of CREB-mediated signaling pathways.	bind
30862	2	9059	6	10	NULL	0	NULL	CBP/p300	NULL		is a type of	NULL				300-kDa protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_8_3697_s_32	9108040	A 300-kDa protein (CBP/p300) which binds to the cAMP response element-binding protein (CREB) functions as a coactivator of CREB-mediated signaling pathways.	bind
30863	3	9059	6	NULL	NULL	0	NULL	CBP/p300	NULL		bind	NULL				CREB	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_94_8_3697_s_32	9108040	A 300-kDa protein (CBP/p300) which binds to the cAMP response element-binding protein (CREB) functions as a coactivator of CREB-mediated signaling pathways.	bind
30864	4	9059	6	NULL	NULL	0	NULL	CBP/p300	NULL		functions as a	NULL				coactivator	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_94_8_3697_s_32	9108040	A 300-kDa protein (CBP/p300) which binds to the cAMP response element-binding protein (CREB) functions as a coactivator of CREB-mediated signaling pathways.	bind
30865	5	9059	6	NULL	NULL	0	NULL	CREB	NULL		mediates	NULL				signaling pathways	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_94_8_3697_s_32	9108040	A 300-kDa protein (CBP/p300) which binds to the cAMP response element-binding protein (CREB) functions as a coactivator of CREB-mediated signaling pathways.	bind
30866	6	9059	6	NULL	NULL	0	NULL	statement 4	NULL		occurs in	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_94_8_3697_s_32	9108040	A 300-kDa protein (CBP/p300) which binds to the cAMP response element-binding protein (CREB) functions as a coactivator of CREB-mediated signaling pathways.	bind
38908	1	9060	5	13	NULL	NULL	NULL	F3 peptide	GP		corresponds to					HMGN2	GP		nucleosomal binding domain		NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_11_7444_s_96	12032302	A 31-aa fragment encoded by exons 3 and 4 (F3 peptide) showed substantial tumor cell binding (Fig.  2); F3 corresponds to the nucleosomal binding domain of HMGN2.	bind
38909	2	9060	5	13	NULL	NULL	NULL	F3 peptide	GP		bind		substantially			tumor cell	Cell				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_11_7444_s_96	12032302	A 31-aa fragment encoded by exons 3 and 4 (F3 peptide) showed substantial tumor cell binding (Fig.  2); F3 corresponds to the nucleosomal binding domain of HMGN2.	bind
47987	3	9060	5	13	NULL	NULL	NULL	F3 peptide	GP		is					31-aa fragment 	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_11_7444_s_96	12032302	A 31-aa fragment encoded by exons 3 and 4 (F3 peptide) showed substantial tumor cell binding (Fig.  2); F3 corresponds to the nucleosomal binding domain of HMGN2.	bind
47988	4	9060	5	13	NULL	NULL	NULL				encodes				exon 3	F3 peptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_11_7444_s_96	12032302	A 31-aa fragment encoded by exons 3 and 4 (F3 peptide) showed substantial tumor cell binding (Fig.  2); F3 corresponds to the nucleosomal binding domain of HMGN2.	bind
47989	5	9060	5	13	NULL	NULL	NULL				encodes				exon 4	F3 peptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_11_7444_s_96	12032302	A 31-aa fragment encoded by exons 3 and 4 (F3 peptide) showed substantial tumor cell binding (Fig.  2); F3 corresponds to the nucleosomal binding domain of HMGN2.	bind
47990	6	9060	5	13	NULL	NULL	NULL	statement 4	Process		occur along with					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_11_7444_s_96	12032302	A 31-aa fragment encoded by exons 3 and 4 (F3 peptide) showed substantial tumor cell binding (Fig.  2); F3 corresponds to the nucleosomal binding domain of HMGN2.	bind
30868	1	9060	6	NULL	NULL	0	NULL	F3 peptide	NULL		corresponds to	NULL				HMGN2	NULL		nucleosomal binding domain		NULL		0	NULL	NULL	NULL	gw60_pnas_99_11_7444_s_96	12032302	A 31-aa fragment encoded by exons 3 and 4 (F3 peptide) showed substantial tumor cell binding (Fig.  2); F3 corresponds to the nucleosomal binding domain of HMGN2.	bind
30870	2	9060	6	NULL	NULL	0	NULL	F3 peptide	NULL		bind	NULL	substantially			tumor cell	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_11_7444_s_96	12032302	A 31-aa fragment encoded by exons 3 and 4 (F3 peptide) showed substantial tumor cell binding (Fig.  2); F3 corresponds to the nucleosomal binding domain of HMGN2.	bind
30871	4	9060	6	10	NULL	0	NULL		NULL		encode	NULL			exon 3	F3 peptide	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_11_7444_s_96	12032302	A 31-aa fragment encoded by exons 3 and 4 (F3 peptide) showed substantial tumor cell binding (Fig.  2); F3 corresponds to the nucleosomal binding domain of HMGN2.	bind
30874	3	9060	6	10	NULL	0	NULL	F3 peptide	NULL		is	NULL				31-aa fragment	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_11_7444_s_96	12032302	A 31-aa fragment encoded by exons 3 and 4 (F3 peptide) showed substantial tumor cell binding (Fig.  2); F3 corresponds to the nucleosomal binding domain of HMGN2.	bind
47991	5	9060	6	10	NULL	0	NULL		NULL		encode	NULL			exon 4	F3 peptide	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_11_7444_s_96	12032302	A 31-aa fragment encoded by exons 3 and 4 (F3 peptide) showed substantial tumor cell binding (Fig.  2); F3 corresponds to the nucleosomal binding domain of HMGN2.	bind
47992	6	9060	6	10	NULL	0	NULL	statement 4	NULL		occur along with	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_11_7444_s_96	12032302	A 31-aa fragment encoded by exons 3 and 4 (F3 peptide) showed substantial tumor cell binding (Fig.  2); F3 corresponds to the nucleosomal binding domain of HMGN2.	bind
38910	1	9061	5	13	NULL	NULL	NULL	double-stranded oligonucleotide probe	NucleicAcid	32P-labeled	contains					ApoJ/lusterin	GP	human;;putative		Myb binding site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_28_21055_s_114	10770937	A 32P-labeled double-stranded oligonucleotide probe containing the putative Myb binding site of the human ApoJ/lusterin promoter bound to GST/B- MYB, but not to GST alone (Fig.  6,  lanes 1 and  2).	bind
38911	2	9061	5	13	NULL	NULL	NULL	statement 1	NucleicAcid		bind					GST/B- MYB	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_28_21055_s_114	10770937	A 32P-labeled double-stranded oligonucleotide probe containing the putative Myb binding site of the human ApoJ/lusterin promoter bound to GST/B- MYB, but not to GST alone (Fig.  6,  lanes 1 and  2).	bind
38912	3	9061	5	13	NULL	NULL	NULL	statement 1	NucleicAcid		does not bind					GST	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_28_21055_s_114	10770937	A 32P-labeled double-stranded oligonucleotide probe containing the putative Myb binding site of the human ApoJ/lusterin promoter bound to GST/B- MYB, but not to GST alone (Fig.  6,  lanes 1 and  2).	bind
30875	1	9061	6	NULL	NULL	0	NULL	ApoJ/lusterin	NULL	32P-labeled;; human;; putative	bind	NULL			Myb binding site of promoter	GST/B- MYB	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_28_21055_s_114	10770937	A 32P-labeled double-stranded oligonucleotide probe containing the putative Myb binding site of the human ApoJ/lusterin promoter bound to GST/B- MYB, but not to GST alone (Fig.  6,  lanes 1 and  2).	bind
30876	2	9061	6	NULL	NULL	0	NULL	ApoJ/lusterin	NULL	32P-labeled;; human;; putative	does not bind	NULL			Myb binding site of promoter	GST	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_28_21055_s_114	10770937	A 32P-labeled double-stranded oligonucleotide probe containing the putative Myb binding site of the human ApoJ/lusterin promoter bound to GST/B- MYB, but not to GST alone (Fig.  6,  lanes 1 and  2).	bind
38986	2	9063	5	13	NULL	NULL	NULL	statement 1	GP		bind					CAM kinase II	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_20_0_253_s_636	11861604	A 33 amino acid  fragment containing residues of the juxta-membrane portion of the cytoplasmic region  of CD5 bound to CAM kinase II .	bind
47993	1	9063	5	13	NULL	NULL	NULL	33 amino acid fragment	GP		contains					CD5	GP		residues of  juxta-membrane portion of the cytoplasmic region 		NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_20_0_253_s_636	11861604	A 33 amino acid  fragment containing residues of the juxta-membrane portion of the cytoplasmic region  of CD5 bound to CAM kinase II .	bind
30877	2	9063	6	10	NULL	0	NULL	statement 1	NULL		bind	NULL				CAM kinase II	NULL				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_20_0_253_s_636	11861604	A 33 amino acid  fragment containing residues of the juxta-membrane portion of the cytoplasmic region  of CD5 bound to CAM kinase II .	bind
47994	1	9063	6	10	NULL	0	NULL	33 amino acid fragment	NULL		contains	NULL				CD5	NULL		residues of the juxta-membrane portion of the cytoplasmic region		NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_20_0_253_s_636	11861604	A 33 amino acid  fragment containing residues of the juxta-membrane portion of the cytoplasmic region  of CD5 bound to CAM kinase II .	bind
38987	1	9064	5	13	NULL	NULL	NULL				encode				exon 1	35-amino-acid-long presequence	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1592_1_63_s_263	12191769	A 35-amino-acid-long presequence is encoded by exon 1, and the entire metal-binding domain by exon 13.	bind
38988	2	9064	5	10	NULL	0	NULL				encode				exon 13				entire metal-binding domain		NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1592_1_63_s_263	12191769	A 35-amino-acid-long presequence is encoded by exon 1, and the entire metal-binding domain by exon 13.	bind
31091	1	9064	6	10	NULL	0	NULL	exon 13			encodes								metal-binding domain		NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1592_1_63_s_263	12191769	A 35-amino-acid-long presequence is encoded by exon 1, and the entire metal-binding domain by exon 13.	bind
31092	2	9064	6	NULL	NULL	0	NULL	exon 1	NULL		encodes	NULL				35-amino-acid-long presequence	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1592_1_63_s_263	12191769	A 35-amino-acid-long presequence is encoded by exon 1, and the entire metal-binding domain by exon 13.	bind
38989	1	9065	5	13	NULL	NULL	NULL	CIITA	GP		inhibit		effectively	36-amino-acid region of 		CBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_42_26562_s_307	9334236	A 36-Amino-Acid Region of CIITA Is an Effective Inhibitor of CBP: Novel Mechanism of Gamma Interferon-Mediated Suppression of Collagen {alpha}2	bind
38990	2	9065	5	13	NULL	NULL	NULL	Gamma Interferon	GP		mediate					Collagen {alpha}2	GP	suppression of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_42_26562_s_307	9334236	A 36-Amino-Acid Region of CIITA Is an Effective Inhibitor of CBP: Novel Mechanism of Gamma Interferon-Mediated Suppression of Collagen {alpha}2	bind
30879	1	9065	6	NULL	NULL	0	NULL	Gamma Interferon	NULL		mediates	NULL				Collagen (alpha)2	NULL	suppression of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_42_26562_s_307	9334236	A 36-Amino-Acid Region of CIITA Is an Effective Inhibitor of CBP: Novel Mechanism of Gamma Interferon-Mediated Suppression of Collagen {alpha}2	bind
30880	2	9065	6	10	NULL	0	NULL	CIITA			inhibits		effectively	36 amino-acid region		CBP					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_42_26562_s_307	9334236	A 36-Amino-Acid Region of CIITA Is an Effective Inhibitor of CBP: Novel Mechanism of Gamma Interferon-Mediated Suppression of Collagen {alpha}2	bind
38991	1	9066	5	13	NULL	NULL	NULL				is purified from			36-kDa N-terminal fragment		liver nuclei	CellComponent	rabbit			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_49_31191_s_31	8940119	A 36-kDa N-terminal fragment was purified from rabbit liver nuclei that could bind GTP, suggesting that the N terminus of tTG plays an important role in nucleotide binding ( 17).	bind
38992	2	9066	5	13	NULL	NULL	NULL	tTG	GP		plays a role in			N terminus		nucleotide	NucleicAcid	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_49_31191_s_31	8940119	A 36-kDa N-terminal fragment was purified from rabbit liver nuclei that could bind GTP, suggesting that the N terminus of tTG plays an important role in nucleotide binding ( 17).	bind
38993	3	9066	5	13	NULL	NULL	NULL	statement 1	Process		suggest					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_49_31191_s_31	8940119	A 36-kDa N-terminal fragment was purified from rabbit liver nuclei that could bind GTP, suggesting that the N terminus of tTG plays an important role in nucleotide binding ( 17).	bind
47995	4	9066	5	13	NULL	NULL	NULL	statement 1	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_49_31191_s_31	8940119	A 36-kDa N-terminal fragment was purified from rabbit liver nuclei that could bind GTP, suggesting that the N terminus of tTG plays an important role in nucleotide binding ( 17).	bind
30881	1	9066	6	NULL	NULL	0	NULL	tTG	NULL		plays an important role in	NULL		N terminus		nucleotide	NULL	binding of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_49_31191_s_31	8940119	A 36-kDa N-terminal fragment was purified from rabbit liver nuclei that could bind GTP, suggesting that the N terminus of tTG plays an important role in nucleotide binding ( 17).	bind
30882	2	9066	6	NULL	NULL	0	NULL	36-kDa	NULL		is purified from	NULL		N-terminal fragment		liver nuclei	NULL	rabbit			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_49_31191_s_31	8940119	A 36-kDa N-terminal fragment was purified from rabbit liver nuclei that could bind GTP, suggesting that the N terminus of tTG plays an important role in nucleotide binding ( 17).	bind
30883	3	9066	6	NULL	NULL	0	NULL	statement 2	NULL		bind	NULL				GTP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_49_31191_s_31	8940119	A 36-kDa N-terminal fragment was purified from rabbit liver nuclei that could bind GTP, suggesting that the N terminus of tTG plays an important role in nucleotide binding ( 17).	bind
30884	4	9066	6	NULL	NULL	0	NULL	statement 3	NULL		suggests	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_49_31191_s_31	8940119	A 36-kDa N-terminal fragment was purified from rabbit liver nuclei that could bind GTP, suggesting that the N terminus of tTG plays an important role in nucleotide binding ( 17).	bind
39527	1	9067	5	13	NULL	NULL	NULL	Mrb-sat23 oligonucleotide	NucleicAcid		contains				38-bp segment			M. rufogriseus		17-bp CENP-B box 	NULL		NULL	NULL	NULL	NULL	gw70_genetics_172_2_1129_s_119	16387881	A 38-bp segment of the Mrb-sat23 oligonucleotide containing the 17-bp  M. rufogriseus CENP-B box ( Figure 1) bound selectively to  M. rufogriseus nuclear protein and shifted upon the addition of human anti-CENP-B (rabbit) antibody ( Figure 4A).	bind
39528	2	9067	5	13	NULL	NULL	NULL	statement 1	NucleicAcid		bind		selectively			nuclear protein	GP	M. rufogriseus			NULL		NULL	NULL	NULL	NULL	gw70_genetics_172_2_1129_s_119	16387881	A 38-bp segment of the Mrb-sat23 oligonucleotide containing the 17-bp  M. rufogriseus CENP-B box ( Figure 1) bound selectively to  M. rufogriseus nuclear protein and shifted upon the addition of human anti-CENP-B (rabbit) antibody ( Figure 4A).	bind
30956	2	9067	6	10	NULL	0	NULL	statement 1	NULL		bind	NULL	selectively			nuclear protein	NULL	M. rufogriseus			NULL		NULL	NULL	NULL	NULL	gw70_genetics_172_2_1129_s_119	16387881	A 38-bp segment of the Mrb-sat23 oligonucleotide containing the 17-bp  M. rufogriseus CENP-B box ( Figure 1) bound selectively to  M. rufogriseus nuclear protein and shifted upon the addition of human anti-CENP-B (rabbit) antibody ( Figure 4A).	bind
31012	1	9067	6	10	NULL	0	NULL	Mrb-sat23 oligonucleotide	NULL		contains	NULL			38-bp segment		NULL	M. rufogriseus		17-bp CENP-B box	NULL		NULL	NULL	NULL	NULL	gw70_genetics_172_2_1129_s_119	16387881	A 38-bp segment of the Mrb-sat23 oligonucleotide containing the 17-bp  M. rufogriseus CENP-B box ( Figure 1) bound selectively to  M. rufogriseus nuclear protein and shifted upon the addition of human anti-CENP-B (rabbit) antibody ( Figure 4A).	bind
38994	2	9068	5	13	NULL	NULL	NULL	statement 1	GP		bind					CD40	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_105_3_301_s_372	10675356	A 39 kDa protein on activated helper T cells binds CD40 and transduces signals to cognate activation of B cells.	bind
38995	3	9068	5	13	NULL	NULL	NULL	statement 2	Process		transduce signal to					B cells	Cell	cognate activation of			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_105_3_301_s_372	10675356	A 39 kDa protein on activated helper T cells binds CD40 and transduces signals to cognate activation of B cells.	bind
47996	1	9068	5	13	NULL	NULL	NULL	39 kDa protein	GP		localized on					helper T cells	Cell	activated			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_105_3_301_s_372	10675356	A 39 kDa protein on activated helper T cells binds CD40 and transduces signals to cognate activation of B cells.	bind
31016	1	9068	6	NULL	NULL	0	NULL	39 kDa protein	NULL		is localized on	NULL				helper T cells	NULL	activated			NULL		0	NULL	NULL	NULL	gw60_jclininvest_105_3_301_s_372	10675356	A 39 kDa protein on activated helper T cells binds CD40 and transduces signals to cognate activation of B cells.	bind
31017	2	9068	6	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL				CD40	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_105_3_301_s_372	10675356	A 39 kDa protein on activated helper T cells binds CD40 and transduces signals to cognate activation of B cells.	bind
31018	3	9068	6	10	NULL	0	NULL	statement 2	NULL		 transduce signals to	NULL				B cells 	NULL	 cognate activation of			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_105_3_301_s_372	10675356	A 39 kDa protein on activated helper T cells binds CD40 and transduces signals to cognate activation of B cells.	bind
38996	1	9072	5	13	NULL	NULL	NULL	RAP	GP		is					receptor-associated protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_16_9543_s_20	7721883	A 39-kDa protein, termed the  receptor-associated protein (RAP) binds to LRP  ( 21) , gp330  ( 22) , and the VLDL receptor   ( 23) with high affinity,  and to the LDL receptor with weaker affinity  ( 24) .	bind
38997	2	9072	5	13	NULL	NULL	NULL	RAP	GP		is a type of					39-kDa protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_16_9543_s_20	7721883	A 39-kDa protein, termed the  receptor-associated protein (RAP) binds to LRP  ( 21) , gp330  ( 22) , and the VLDL receptor   ( 23) with high affinity,  and to the LDL receptor with weaker affinity  ( 24) .	bind
38998	3	9072	5	13	NULL	NULL	NULL	RAP	GP		bind		high affinity			LRP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_16_9543_s_20	7721883	A 39-kDa protein, termed the  receptor-associated protein (RAP) binds to LRP  ( 21) , gp330  ( 22) , and the VLDL receptor   ( 23) with high affinity,  and to the LDL receptor with weaker affinity  ( 24) .	bind
38999	4	9072	5	13	NULL	NULL	NULL	RAP	GP		bind		high affinity			gp330	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_16_9543_s_20	7721883	A 39-kDa protein, termed the  receptor-associated protein (RAP) binds to LRP  ( 21) , gp330  ( 22) , and the VLDL receptor   ( 23) with high affinity,  and to the LDL receptor with weaker affinity  ( 24) .	bind
39000	5	9072	5	13	NULL	NULL	NULL	RAP	GP		bind		high affinity			VLDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_16_9543_s_20	7721883	A 39-kDa protein, termed the  receptor-associated protein (RAP) binds to LRP  ( 21) , gp330  ( 22) , and the VLDL receptor   ( 23) with high affinity,  and to the LDL receptor with weaker affinity  ( 24) .	bind
39001	6	9072	5	13	NULL	NULL	NULL	RAP	GP		bind		weak affinity			LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_16_9543_s_20	7721883	A 39-kDa protein, termed the  receptor-associated protein (RAP) binds to LRP  ( 21) , gp330  ( 22) , and the VLDL receptor   ( 23) with high affinity,  and to the LDL receptor with weaker affinity  ( 24) .	bind
31019	1	9072	6	NULL	NULL	0	NULL	RAP	NULL		bind	NULL	high affinity			LRP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_16_9543_s_20	7721883	A 39-kDa protein, termed the  receptor-associated protein (RAP) binds to LRP  ( 21) , gp330  ( 22) , and the VLDL receptor   ( 23) with high affinity,  and to the LDL receptor with weaker affinity  ( 24) .	bind
31020	2	9072	6	NULL	NULL	0	NULL	RAP	NULL		is	NULL				receptor-associated protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_16_9543_s_20	7721883	A 39-kDa protein, termed the  receptor-associated protein (RAP) binds to LRP  ( 21) , gp330  ( 22) , and the VLDL receptor   ( 23) with high affinity,  and to the LDL receptor with weaker affinity  ( 24) .	bind
31021	3	9072	6	10	NULL	0	NULL	RAP	NULL		is a type of	NULL				39-kDa protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_16_9543_s_20	7721883	A 39-kDa protein, termed the  receptor-associated protein (RAP) binds to LRP  ( 21) , gp330  ( 22) , and the VLDL receptor   ( 23) with high affinity,  and to the LDL receptor with weaker affinity  ( 24) .	bind
31022	4	9072	6	NULL	NULL	0	NULL	RAP	NULL		bind	NULL	high affinity			gp330	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_16_9543_s_20	7721883	A 39-kDa protein, termed the  receptor-associated protein (RAP) binds to LRP  ( 21) , gp330  ( 22) , and the VLDL receptor   ( 23) with high affinity,  and to the LDL receptor with weaker affinity  ( 24) .	bind
31023	5	9072	6	NULL	NULL	0	NULL	RAP	NULL		bind	NULL	high affinity			VLDL receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_16_9543_s_20	7721883	A 39-kDa protein, termed the  receptor-associated protein (RAP) binds to LRP  ( 21) , gp330  ( 22) , and the VLDL receptor   ( 23) with high affinity,  and to the LDL receptor with weaker affinity  ( 24) .	bind
31024	6	9072	6	NULL	NULL	0	NULL	RAP	NULL		bind	NULL	weak affinity			LDL receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_16_9543_s_20	7721883	A 39-kDa protein, termed the  receptor-associated protein (RAP) binds to LRP  ( 21) , gp330  ( 22) , and the VLDL receptor   ( 23) with high affinity,  and to the LDL receptor with weaker affinity  ( 24) .	bind
39002	1	9073	5	13	NULL	NULL	NULL	RAP	GP		is a type of					39-kDa receptor-associated protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_53_37685_s_44	10608826	A 39-kDa receptor-associated protein (RAP) binds to LRP with high affinity ( K d = 4 nM ( 27)) and inhibits binding and LRP-mediated internalization and degradation of all ligands ( 30,  33), therefore serving as a useful tool for testing whether LRP is involved in endocytosis of a given ligand.	bind
39003	2	9073	5	13	NULL	NULL	NULL	RAP	GP		bind		high affinity			LRP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_53_37685_s_44	10608826	A 39-kDa receptor-associated protein (RAP) binds to LRP with high affinity ( K d = 4 nM ( 27)) and inhibits binding and LRP-mediated internalization and degradation of all ligands ( 30,  33), therefore serving as a useful tool for testing whether LRP is involved in endocytosis of a given ligand.	bind
39004	3	9073	5	13	NULL	NULL	NULL	statement 2	Process		inhibit					ligand	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_53_37685_s_44	10608826	A 39-kDa receptor-associated protein (RAP) binds to LRP with high affinity ( K d = 4 nM ( 27)) and inhibits binding and LRP-mediated internalization and degradation of all ligands ( 30,  33), therefore serving as a useful tool for testing whether LRP is involved in endocytosis of a given ligand.	bind
39005	4	9073	5	13	NULL	NULL	NULL	LRP	GP		mediate					ligand	GP	internalization of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_53_37685_s_44	10608826	A 39-kDa receptor-associated protein (RAP) binds to LRP with high affinity ( K d = 4 nM ( 27)) and inhibits binding and LRP-mediated internalization and degradation of all ligands ( 30,  33), therefore serving as a useful tool for testing whether LRP is involved in endocytosis of a given ligand.	bind
39006	5	9073	5	13	NULL	NULL	NULL	LRP	GP		mediate					ligand	GP	degradation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_53_37685_s_44	10608826	A 39-kDa receptor-associated protein (RAP) binds to LRP with high affinity ( K d = 4 nM ( 27)) and inhibits binding and LRP-mediated internalization and degradation of all ligands ( 30,  33), therefore serving as a useful tool for testing whether LRP is involved in endocytosis of a given ligand.	bind
39007	6	9073	5	13	NULL	NULL	NULL	statement 2	Process		inhibit					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_53_37685_s_44	10608826	A 39-kDa receptor-associated protein (RAP) binds to LRP with high affinity ( K d = 4 nM ( 27)) and inhibits binding and LRP-mediated internalization and degradation of all ligands ( 30,  33), therefore serving as a useful tool for testing whether LRP is involved in endocytosis of a given ligand.	bind
39008	7	9073	5	13	NULL	NULL	NULL	statement 2	Process		inhibit					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_53_37685_s_44	10608826	A 39-kDa receptor-associated protein (RAP) binds to LRP with high affinity ( K d = 4 nM ( 27)) and inhibits binding and LRP-mediated internalization and degradation of all ligands ( 30,  33), therefore serving as a useful tool for testing whether LRP is involved in endocytosis of a given ligand.	bind
47997	8	9073	5	13	NULL	NULL	NULL	RAP	GP		is					receptor-associated protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_53_37685_s_44	10608826	A 39-kDa receptor-associated protein (RAP) binds to LRP with high affinity ( K d = 4 nM ( 27)) and inhibits binding and LRP-mediated internalization and degradation of all ligands ( 30,  33), therefore serving as a useful tool for testing whether LRP is involved in endocytosis of a given ligand.	bind
31025	1	9073	6	NULL	NULL	0	NULL	RAP	NULL		bind	NULL	high affinity			LRP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_53_37685_s_44	10608826	A 39-kDa receptor-associated protein (RAP) binds to LRP with high affinity ( K d = 4 nM ( 27)) and inhibits binding and LRP-mediated internalization and degradation of all ligands ( 30,  33), therefore serving as a useful tool for testing whether LRP is involved in endocytosis of a given ligand.	bind
31026	2	9073	6	NULL	NULL	0	NULL	RAP	NULL		is	NULL				receptor-associated protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_53_37685_s_44	10608826	A 39-kDa receptor-associated protein (RAP) binds to LRP with high affinity ( K d = 4 nM ( 27)) and inhibits binding and LRP-mediated internalization and degradation of all ligands ( 30,  33), therefore serving as a useful tool for testing whether LRP is involved in endocytosis of a given ligand.	bind
31027	3	9073	6	10	NULL	0	NULL	RAP	NULL		is a type of	NULL				39-kDa protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_53_37685_s_44	10608826	A 39-kDa receptor-associated protein (RAP) binds to LRP with high affinity ( K d = 4 nM ( 27)) and inhibits binding and LRP-mediated internalization and degradation of all ligands ( 30,  33), therefore serving as a useful tool for testing whether LRP is involved in endocytosis of a given ligand.	bind
31028	4	9073	6	NULL	NULL	0	NULL	LRP	NULL		mediates	NULL				ligands	NULL	internalization of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_53_37685_s_44	10608826	A 39-kDa receptor-associated protein (RAP) binds to LRP with high affinity ( K d = 4 nM ( 27)) and inhibits binding and LRP-mediated internalization and degradation of all ligands ( 30,  33), therefore serving as a useful tool for testing whether LRP is involved in endocytosis of a given ligand.	bind
31029	5	9073	6	NULL	NULL	0	NULL	LRP	NULL		mediates	NULL				ligands	NULL	degradation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_53_37685_s_44	10608826	A 39-kDa receptor-associated protein (RAP) binds to LRP with high affinity ( K d = 4 nM ( 27)) and inhibits binding and LRP-mediated internalization and degradation of all ligands ( 30,  33), therefore serving as a useful tool for testing whether LRP is involved in endocytosis of a given ligand.	bind
31030	6	9073	6	NULL	NULL	0	NULL	RAP	NULL		inhibits	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_53_37685_s_44	10608826	A 39-kDa receptor-associated protein (RAP) binds to LRP with high affinity ( K d = 4 nM ( 27)) and inhibits binding and LRP-mediated internalization and degradation of all ligands ( 30,  33), therefore serving as a useful tool for testing whether LRP is involved in endocytosis of a given ligand.	bind
31031	7	9073	6	NULL	NULL	0	NULL	RAP	NULL		inhibits	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_53_37685_s_44	10608826	A 39-kDa receptor-associated protein (RAP) binds to LRP with high affinity ( K d = 4 nM ( 27)) and inhibits binding and LRP-mediated internalization and degradation of all ligands ( 30,  33), therefore serving as a useful tool for testing whether LRP is involved in endocytosis of a given ligand.	bind
31032	8	9073	6	NULL	NULL	0	NULL	RAP	NULL		inhibits	NULL				ligands	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_53_37685_s_44	10608826	A 39-kDa receptor-associated protein (RAP) binds to LRP with high affinity ( K d = 4 nM ( 27)) and inhibits binding and LRP-mediated internalization and degradation of all ligands ( 30,  33), therefore serving as a useful tool for testing whether LRP is involved in endocytosis of a given ligand.	bind
39010	1	9076	5	13	NULL	NULL	NULL	LPL	GP		bind					ECM	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_3_1329_s_100	8576120	A 4-fold excess of Cu-OxLDL was also able to  abolish the interaction of  I-LDL (12.5 mug/ml) with  LPL bound to the ECM ( Fig. 5).	bind
39011	2	9076	5	13	NULL	NULL	NULL	I-LDL	GP		interact with					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_3_1329_s_100	8576120	A 4-fold excess of Cu-OxLDL was also able to  abolish the interaction of  I-LDL (12.5 mug/ml) with  LPL bound to the ECM ( Fig. 5).	bind
39012	3	9076	5	13	NULL	NULL	NULL	Cu-OxLDL	GP	excess	abolishes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_3_1329_s_100	8576120	A 4-fold excess of Cu-OxLDL was also able to  abolish the interaction of  I-LDL (12.5 mug/ml) with  LPL bound to the ECM ( Fig. 5).	bind
31033	1	9076	6	NULL	NULL	0	NULL	LPL	NULL		bind	NULL				ECM	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_3_1329_s_100	8576120	A 4-fold excess of Cu-OxLDL was also able to  abolish the interaction of  I-LDL (12.5 mug/ml) with  LPL bound to the ECM ( Fig. 5).	bind
31034	2	9076	6	NULL	NULL	0	NULL	I-LDL	NULL		interacts with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_3_1329_s_100	8576120	A 4-fold excess of Cu-OxLDL was also able to  abolish the interaction of  I-LDL (12.5 mug/ml) with  LPL bound to the ECM ( Fig. 5).	bind
31035	3	9076	6	NULL	NULL	0	NULL	Cu-OxLDL	NULL	excess of	abolish	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_3_1329_s_100	8576120	A 4-fold excess of Cu-OxLDL was also able to  abolish the interaction of  I-LDL (12.5 mug/ml) with  LPL bound to the ECM ( Fig. 5).	bind
39013	1	9077	5	13	NULL	NULL	NULL	T cells	Cell	activated	bind					CHO-B7h cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_immunity_11_4_423_s_135	10549624	A 4-fold greater number of activated T cells bound to CHO-B7h cells over CHO-GFP cells (  Figure 4C).	bind
39014	2	9077	5	13	NULL	NULL	NULL	T cells	Cell	activated	bind					CHO-GFP cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_immunity_11_4_423_s_135	10549624	A 4-fold greater number of activated T cells bound to CHO-B7h cells over CHO-GFP cells (  Figure 4C).	bind
39015	3	9077	5	13	NULL	NULL	NULL	statement 1	Process		greater than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_11_4_423_s_135	10549624	A 4-fold greater number of activated T cells bound to CHO-B7h cells over CHO-GFP cells (  Figure 4C).	bind
31036	1	9077	6	NULL	NULL	0	NULL	T cells	NULL	activated	bind	NULL				CHO-B7h cells	NULL				NULL		0	NULL	NULL	NULL	gw60_immunity_11_4_423_s_135	10549624	A 4-fold greater number of activated T cells bound to CHO-B7h cells over CHO-GFP cells (  Figure 4C).	bind
31039	2	9077	6	NULL	NULL	0	NULL	T cells	NULL	activated	bind	NULL				CHO-GFP cells	NULL				NULL		0	NULL	NULL	NULL	gw60_immunity_11_4_423_s_135	10549624	A 4-fold greater number of activated T cells bound to CHO-B7h cells over CHO-GFP cells (  Figure 4C).	bind
31041	3	9077	6	10	NULL	0	NULL	statement 1	NULL	affinity of	is more than	NULL				statement 2	NULL	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_immunity_11_4_423_s_135	10549624	A 4-fold greater number of activated T cells bound to CHO-B7h cells over CHO-GFP cells (  Figure 4C).	bind
39016	1	9078	5	13	NULL	NULL	NULL	AP2	GP		bind					VEGF	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24602_s_200	16790435	A 4-fold induction of AP2 binding to the VEGF promoter region was observed following PGE2 treatment, whereas PGE2 doubled the binding of Sp1 to the VEGF promoter.	bind
39017	2	9078	5	13	NULL	NULL	NULL	PGE2	Chemical		induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24602_s_200	16790435	A 4-fold induction of AP2 binding to the VEGF promoter region was observed following PGE2 treatment, whereas PGE2 doubled the binding of Sp1 to the VEGF promoter.	bind
39018	3	9078	5	13	NULL	NULL	NULL	Sp1	GP		bind					VEGF	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24602_s_200	16790435	A 4-fold induction of AP2 binding to the VEGF promoter region was observed following PGE2 treatment, whereas PGE2 doubled the binding of Sp1 to the VEGF promoter.	bind
39019	4	9078	5	13	NULL	NULL	NULL	PGE2	Chemical		increase					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24602_s_200	16790435	A 4-fold induction of AP2 binding to the VEGF promoter region was observed following PGE2 treatment, whereas PGE2 doubled the binding of Sp1 to the VEGF promoter.	bind
57761	5	9078	5	13	NULL	NULL	NULL	statement 2	Process	induction of	is higher than					statement 4	Process	induction of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24602_s_200	16790435	A 4-fold induction of AP2 binding to the VEGF promoter region was observed following PGE2 treatment, whereas PGE2 doubled the binding of Sp1 to the VEGF promoter.	bind
31042	1	9078	6	NULL	NULL	0	NULL	AP2	NULL		bind	NULL				VEGF	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_34_24602_s_200	16790435	A 4-fold induction of AP2 binding to the VEGF promoter region was observed following PGE2 treatment, whereas PGE2 doubled the binding of Sp1 to the VEGF promoter.	bind
31043	2	9078	6	NULL	NULL	0	NULL	PGE2	NULL		induces	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24602_s_200	16790435	A 4-fold induction of AP2 binding to the VEGF promoter region was observed following PGE2 treatment, whereas PGE2 doubled the binding of Sp1 to the VEGF promoter.	bind
31045	3	9078	6	NULL	NULL	0	NULL	Sp1	NULL		bind	NULL				VEGF	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_34_24602_s_200	16790435	A 4-fold induction of AP2 binding to the VEGF promoter region was observed following PGE2 treatment, whereas PGE2 doubled the binding of Sp1 to the VEGF promoter.	bind
31046	4	9078	6	NULL	NULL	0	NULL	PGE2	NULL		induces	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24602_s_200	16790435	A 4-fold induction of AP2 binding to the VEGF promoter region was observed following PGE2 treatment, whereas PGE2 doubled the binding of Sp1 to the VEGF promoter.	bind
31151	5	9078	6	10	NULL	0	NULL	statement 2		induction of	is higher than					statement 4		induction of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24602_s_200	16790435	A 4-fold induction of AP2 binding to the VEGF promoter region was observed following PGE2 treatment, whereas PGE2 doubled the binding of Sp1 to the VEGF promoter.	bind
39167	1	9080	5	13	NULL	NULL	NULL	NE proteins	GP		bind				A3 Enhancer	A3 RNA	NucleicAcid	biotinylated			NULL		NULL	NULL	NULL	NULL	gw60_cell_93_1_139_s_50	9546399	A 40 kDa SR Protein  Binds Specifically to the A3 Enhancer NE proteins bound to biotinylated A3 (lane  1) or S3 (lane 2) RNA were resolved by 9% SDS/PAGE and analyzed by Western  blot with mAb104.	bind
47998	5	9080	5	13	NULL	NULL	NULL	SR protein	GP		bind		specifically			statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_93_1_139_s_50	9546399	A 40 kDa SR Protein  Binds Specifically to the A3 Enhancer NE proteins bound to biotinylated A3 (lane  1) or S3 (lane 2) RNA were resolved by 9% SDS/PAGE and analyzed by Western  blot with mAb104.	bind
47999	2	9080	5	13	NULL	NULL	NULL	NE proteins	GP		bind				A3 Enhancer	S3 RNA	NucleicAcid	biotinylated			NULL		NULL	NULL	NULL	NULL	gw60_cell_93_1_139_s_50	9546399	A 40 kDa SR Protein  Binds Specifically to the A3 Enhancer NE proteins bound to biotinylated A3 (lane  1) or S3 (lane 2) RNA were resolved by 9% SDS/PAGE and analyzed by Western  blot with mAb104.	bind
48000	3	9080	5	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_93_1_139_s_50	9546399	A 40 kDa SR Protein  Binds Specifically to the A3 Enhancer NE proteins bound to biotinylated A3 (lane  1) or S3 (lane 2) RNA were resolved by 9% SDS/PAGE and analyzed by Western  blot with mAb104.	bind
48001	4	9080	5	13	NULL	NULL	NULL	SR protein	GP		is a type of					40 kDa protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_93_1_139_s_50	9546399	A 40 kDa SR Protein  Binds Specifically to the A3 Enhancer NE proteins bound to biotinylated A3 (lane  1) or S3 (lane 2) RNA were resolved by 9% SDS/PAGE and analyzed by Western  blot with mAb104.	bind
48002	6	9080	5	13	NULL	NULL	NULL	SR protein	GP		bind		specifically			statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_93_1_139_s_50	9546399	A 40 kDa SR Protein  Binds Specifically to the A3 Enhancer NE proteins bound to biotinylated A3 (lane  1) or S3 (lane 2) RNA were resolved by 9% SDS/PAGE and analyzed by Western  blot with mAb104.	bind
31072	1	9080	6	10	NULL	0	NULL	SR protein	NULL		is a type of	NULL				40 kDa protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cell_93_1_139_s_50	9546399	A 40 kDa SR Protein  Binds Specifically to the A3 Enhancer NE proteins bound to biotinylated A3 (lane  1) or S3 (lane 2) RNA were resolved by 9% SDS/PAGE and analyzed by Western  blot with mAb104.	bind
31074	2	9080	6	NULL	NULL	0	NULL	A3 NE proteins	NULL		bind	NULL			enhancer	A3 RNA	NULL	biotinylated			NULL		NULL	NULL	NULL	NULL	gw60_cell_93_1_139_s_50	9546399	A 40 kDa SR Protein  Binds Specifically to the A3 Enhancer NE proteins bound to biotinylated A3 (lane  1) or S3 (lane 2) RNA were resolved by 9% SDS/PAGE and analyzed by Western  blot with mAb104.	bind
31077	3	9080	6	NULL	NULL	0	NULL	A3 NE proteins	NULL		bind	NULL			enhancer	S3 RNA	NULL	biotinylated			NULL		0	NULL	NULL	NULL	gw60_cell_93_1_139_s_50	9546399	A 40 kDa SR Protein  Binds Specifically to the A3 Enhancer NE proteins bound to biotinylated A3 (lane  1) or S3 (lane 2) RNA were resolved by 9% SDS/PAGE and analyzed by Western  blot with mAb104.	bind
31078	4	9080	6	NULL	NULL	0	NULL	statement 2	NULL		is an alternative to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_93_1_139_s_50	9546399	A 40 kDa SR Protein  Binds Specifically to the A3 Enhancer NE proteins bound to biotinylated A3 (lane  1) or S3 (lane 2) RNA were resolved by 9% SDS/PAGE and analyzed by Western  blot with mAb104.	bind
31080	5	9080	6	NULL	NULL	0	NULL	SR protein	NULL		bind	NULL	specifically			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_93_1_139_s_50	9546399	A 40 kDa SR Protein  Binds Specifically to the A3 Enhancer NE proteins bound to biotinylated A3 (lane  1) or S3 (lane 2) RNA were resolved by 9% SDS/PAGE and analyzed by Western  blot with mAb104.	bind
31081	6	9080	6	NULL	NULL	0	NULL	SR protein	NULL		bind	NULL	specifically			statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_93_1_139_s_50	9546399	A 40 kDa SR Protein  Binds Specifically to the A3 Enhancer NE proteins bound to biotinylated A3 (lane  1) or S3 (lane 2) RNA were resolved by 9% SDS/PAGE and analyzed by Western  blot with mAb104.	bind
39166	1	9081	5	13	NULL	NULL	NULL	cytochrome aa3	GP		bind					40-kDa carbon monoxide	Chemical				NULL	Halobacterium halobium membranes	NULL	NULL	NULL	NULL	gw60_jbacteriol_184_3_840_s_151	11790755	A 40-kDa carbon monoxide binding cytochrome  aa3 was previously purified from  Halobacterium halobium membranes.	bind
31183	1	9081	6	10	NULL	0	NULL	cytochrome aa3	NULL		bind	NULL				40-kDa carbon monoxide	NULL				NULL	Halobacterium halobium membranes	NULL	NULL	NULL	NULL	gw60_jbacteriol_184_3_840_s_151	11790755	A 40-kDa carbon monoxide binding cytochrome  aa3 was previously purified from  Halobacterium halobium membranes.	bind
39171	1	9083	5	13	NULL	NULL	NULL	GABA	GP		saturate								GABA binding sites		NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_21_23_9083_s_167	11717341	A 400 msec pulse of 1 mM GABA presumably saturated all of the GABA binding sites.	bind
31184	1	9083	6	10	NULL	0	NULL	GABA	NULL		saturate	NULL					NULL		GABA binding sites		NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_21_23_9083_s_167	11717341	A 400 msec pulse of 1 mM GABA presumably saturated all of the GABA binding sites.	bind
39172	1	9084	5	13	NULL	NULL	NULL	importin alpha	GP		bind			41 amino acid motif		importin beta	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_2_255_s_469	10209022	A 41 amino  acid motif in importin alpha confers binding to importin beta and hence  transit into the nucleus.	bind
39173	2	9084	5	13	NULL	NULL	NULL	statement 1	Process		transit into					nucleus	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_2_255_s_469	10209022	A 41 amino  acid motif in importin alpha confers binding to importin beta and hence  transit into the nucleus.	bind
57762	3	9084	5	13	NULL	NULL	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_2_255_s_469	10209022	A 41 amino  acid motif in importin alpha confers binding to importin beta and hence  transit into the nucleus.	bind
31185	1	9084	6	NULL	NULL	0	NULL	importin alpha	NULL		bind	NULL		41 amino acid		importin beta	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_2_255_s_469	10209022	A 41 amino  acid motif in importin alpha confers binding to importin beta and hence  transit into the nucleus.	bind
31186	2	9084	6	NULL	NULL	0	NULL	importin alpha	NULL		transits into	NULL				nucleus	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_2_255_s_469	10209022	A 41 amino  acid motif in importin alpha confers binding to importin beta and hence  transit into the nucleus.	bind
31187	3	9084	6	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_2_255_s_469	10209022	A 41 amino  acid motif in importin alpha confers binding to importin beta and hence  transit into the nucleus.	bind
39174	1	9089	5	13	NULL	NULL	NULL	importin	GP		bind			41 amino acid motif		importin beta	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_86_6_985_s_346	8808633	A 41 amino acid motif in importin   confers binding to importin beta and hence transit into the nucleus.	bind
39175	2	9089	5	13	NULL	NULL	NULL	statement 1	Process		transit into					nucleus	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cell_86_6_985_s_346	8808633	A 41 amino acid motif in importin   confers binding to importin beta and hence transit into the nucleus.	bind
57763	3	9089	5	13	NULL	NULL	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_86_6_985_s_346	8808633	A 41 amino acid motif in importin   confers binding to importin beta and hence transit into the nucleus.	bind
31188	1	9089	6	NULL	NULL	0	NULL	importin	NULL		bind	NULL		41 amino acid motif		importin beta	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_86_6_985_s_346	8808633	A 41 amino acid motif in importin   confers binding to importin beta and hence transit into the nucleus.	bind
31189	2	9089	6	NULL	NULL	0	NULL	importin	NULL		transits into	NULL				nucleus	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_86_6_985_s_346	8808633	A 41 amino acid motif in importin   confers binding to importin beta and hence transit into the nucleus.	bind
31190	3	9089	6	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_86_6_985_s_346	8808633	A 41 amino acid motif in importin   confers binding to importin beta and hence transit into the nucleus.	bind
39176	1	9097	5	13	NULL	NULL	NULL	45-kDa protein	GP	yeast	is a homolog of			N-terminal		CyP-40	GP	mammalian			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20479_s_28	7657624	A 45-kDa yeast protein with N-terminal  homology to mammalian CyP-40 has been isolated in a multiprotein  complex with the yeast homolog of hsp90 ( 27) , and incubation  of a variety of tissue homogenates with a CyP-40/GST-fusion protein  bound to glutathione-agarose resulted in retention of hsp90,   suggesting that CyP-40 also binds directly to hsp90.	bind
39177	2	9097	5	13	NULL	NULL	NULL	statement 1	GP		is in complex with					 hsp90	GP	yeast homolog of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20479_s_28	7657624	A 45-kDa yeast protein with N-terminal  homology to mammalian CyP-40 has been isolated in a multiprotein  complex with the yeast homolog of hsp90 ( 27) , and incubation  of a variety of tissue homogenates with a CyP-40/GST-fusion protein  bound to glutathione-agarose resulted in retention of hsp90,   suggesting that CyP-40 also binds directly to hsp90.	bind
39178	3	9097	5	13	NULL	NULL	NULL	CyP-40	GP		bind		directly			hsp90	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20479_s_28	7657624	A 45-kDa yeast protein with N-terminal  homology to mammalian CyP-40 has been isolated in a multiprotein  complex with the yeast homolog of hsp90 ( 27) , and incubation  of a variety of tissue homogenates with a CyP-40/GST-fusion protein  bound to glutathione-agarose resulted in retention of hsp90,   suggesting that CyP-40 also binds directly to hsp90.	bind
32022	1	9097	6	NULL	NULL	0	NULL	CyP-40	NULL		bind	NULL	directly			hsp90	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20479_s_28	7657624	A 45-kDa yeast protein with N-terminal  homology to mammalian CyP-40 has been isolated in a multiprotein  complex with the yeast homolog of hsp90 ( 27) , and incubation  of a variety of tissue homogenates with a CyP-40/GST-fusion protein  bound to glutathione-agarose resulted in retention of hsp90,   suggesting that CyP-40 also binds directly to hsp90.	bind
48003	2	9097	6	10	NULL	0	NULL	 45-kDa protein	NULL	yeast	is a homolog of	NULL		N-terminal		CyP-40	NULL	mammalian			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20479_s_28	7657624	A 45-kDa yeast protein with N-terminal  homology to mammalian CyP-40 has been isolated in a multiprotein  complex with the yeast homolog of hsp90 ( 27) , and incubation  of a variety of tissue homogenates with a CyP-40/GST-fusion protein  bound to glutathione-agarose resulted in retention of hsp90,   suggesting that CyP-40 also binds directly to hsp90.	bind
57764	3	9097	6	10	NULL	0	NULL	statement 2			is in complex with					hsp90		yeast homolog of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20479_s_28	7657624	A 45-kDa yeast protein with N-terminal  homology to mammalian CyP-40 has been isolated in a multiprotein  complex with the yeast homolog of hsp90 ( 27) , and incubation  of a variety of tissue homogenates with a CyP-40/GST-fusion protein  bound to glutathione-agarose resulted in retention of hsp90,   suggesting that CyP-40 also binds directly to hsp90.	bind
39179	1	9099	5	13	NULL	NULL	NULL	 Nox	GP	Escherichia coli	bind		noncovalently			FAD	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_24_7007_s_38	11717257	A 47-kDa Nox from  Escherichia coli has a noncovalently bound flavin adenine dinucleotide (FAD) that catalyzes the reduction of a quinone, probably ubiquinone-8, in vivo ( 27).	bind
39180	2	9099	5	13	NULL	NULL	NULL	FAD	NucleicAcid		is					flavin adenine dinucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_24_7007_s_38	11717257	A 47-kDa Nox from  Escherichia coli has a noncovalently bound flavin adenine dinucleotide (FAD) that catalyzes the reduction of a quinone, probably ubiquinone-8, in vivo ( 27).	bind
39181	3	9099	5	13	NULL	NULL	NULL	FAD	NucleicAcid		catalyze					ubiquinone-8	Chemical	reduction of			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbacteriol_183_24_7007_s_38	11717257	A 47-kDa Nox from  Escherichia coli has a noncovalently bound flavin adenine dinucleotide (FAD) that catalyzes the reduction of a quinone, probably ubiquinone-8, in vivo ( 27).	bind
39182	4	9099	5	13	NULL	NULL	NULL	ubiquinone-8	Chemical		is a type of					quinone	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_24_7007_s_38	11717257	A 47-kDa Nox from  Escherichia coli has a noncovalently bound flavin adenine dinucleotide (FAD) that catalyzes the reduction of a quinone, probably ubiquinone-8, in vivo ( 27).	bind
39183	5	9099	5	13	NULL	NULL	NULL	Nox	GP		is a type of					 47-kDa protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_24_7007_s_38	11717257	A 47-kDa Nox from  Escherichia coli has a noncovalently bound flavin adenine dinucleotide (FAD) that catalyzes the reduction of a quinone, probably ubiquinone-8, in vivo ( 27).	bind
31191	1	9099	6	10	NULL	0	NULL	Nox	NULL	Escherichia coli	bind	NULL	noncovalently			FAD	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_24_7007_s_38	11717257	A 47-kDa Nox from  Escherichia coli has a noncovalently bound flavin adenine dinucleotide (FAD) that catalyzes the reduction of a quinone, probably ubiquinone-8, in vivo ( 27).	bind
31192	2	9099	6	NULL	NULL	0	NULL	FAD	NULL		is	NULL				flavin adenine dinucleotide 	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_24_7007_s_38	11717257	A 47-kDa Nox from  Escherichia coli has a noncovalently bound flavin adenine dinucleotide (FAD) that catalyzes the reduction of a quinone, probably ubiquinone-8, in vivo ( 27).	bind
31193	3	9099	6	NULL	NULL	0	NULL	ubiquinone-8	NULL		is a type of	NULL				quinone	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_24_7007_s_38	11717257	A 47-kDa Nox from  Escherichia coli has a noncovalently bound flavin adenine dinucleotide (FAD) that catalyzes the reduction of a quinone, probably ubiquinone-8, in vivo ( 27).	bind
31194	4	9099	6	NULL	NULL	0	NULL	FAD	NULL		catalyzes	NULL				ubiquinone-8	NULL	reduction of 			NULL	in vivo	0	NULL	NULL	NULL	gw60_jbacteriol_183_24_7007_s_38	11717257	A 47-kDa Nox from  Escherichia coli has a noncovalently bound flavin adenine dinucleotide (FAD) that catalyzes the reduction of a quinone, probably ubiquinone-8, in vivo ( 27).	bind
31271	5	9099	6	10	NULL	0	NULL	Nox	NULL		is a type of	NULL				47-kDa protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_24_7007_s_38	11717257	A 47-kDa Nox from  Escherichia coli has a noncovalently bound flavin adenine dinucleotide (FAD) that catalyzes the reduction of a quinone, probably ubiquinone-8, in vivo ( 27).	bind
39184	1	9101	5	13	NULL	NULL	NULL	PAK-1	GP		bind		specifically			cdc42	GP	active			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_14_2821_s_273	15241473	A 5 mug portion of PAK-1 agarose beads, which specifically bound to active cdc42, was added  to the cell lysates and incubated for 1 h at 4 degrees C.	bind
31272	1	9101	6	NULL	NULL	0	NULL	PAK-1	NULL		bind	NULL	specifically			cdc42	NULL	active			NULL		0	NULL	NULL	NULL	gw70_embo_23_14_2821_s_273	15241473	A 5 mug portion of PAK-1 agarose beads, which specifically bound to active cdc42, was added  to the cell lysates and incubated for 1 h at 4 degrees C.	bind
39186	1	9102	5	13	NULL	NULL	NULL	Nanog	GP		regulates				Oct-4 binding sites in promoter	Nanog gene	GP	transcriptional activity of			NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_cell-res_16_3_16541131_s_3	16541131	A 5' flank sequence of the Nanog gene has been  reported to be regulated differentially, and two regulatory elements within  the Nanog promoter, namely Oct-4 and Sox-2 binding sites, have been identified  to regulate the transcriptional activity of Nanog gene.	bind
39187	2	9102	5	13	NULL	NULL	NULL	Nanog	GP		regulates				Sox-2 binding sites in promoter	Nanog gene	GP	transcriptional activity of			NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_cell-res_16_3_16541131_s_3	16541131	A 5' flank sequence of the Nanog gene has been  reported to be regulated differentially, and two regulatory elements within  the Nanog promoter, namely Oct-4 and Sox-2 binding sites, have been identified  to regulate the transcriptional activity of Nanog gene.	bind
39188	3	9102	5	13	NULL	NULL	NULL	Oct-4 binding sites	GP		is a type of					Nanog	GP			regulatory elements within  promoter	NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_cell-res_16_3_16541131_s_3	16541131	A 5' flank sequence of the Nanog gene has been  reported to be regulated differentially, and two regulatory elements within  the Nanog promoter, namely Oct-4 and Sox-2 binding sites, have been identified  to regulate the transcriptional activity of Nanog gene.	bind
39189	4	9102	5	13	NULL	NULL	NULL	Sox-2 binding sites	GP		is a type of					Nanog	GP			regulatory elements within  promoter	NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_cell-res_16_3_16541131_s_3	16541131	A 5' flank sequence of the Nanog gene has been  reported to be regulated differentially, and two regulatory elements within  the Nanog promoter, namely Oct-4 and Sox-2 binding sites, have been identified  to regulate the transcriptional activity of Nanog gene.	bind
31273	1	9102	6	NULL	NULL	0	NULL	Nanog	NULL		regulate	NULL			Oct-4 binding site of promoter	Nanog gene	NULL	transcriptional activity of 			NULL		0	NULL	NULL	NULL	abs-batch0620-0649_cell-res_16_3_16541131_s_3	16541131	A 5' flank sequence of the Nanog gene has been  reported to be regulated differentially, and two regulatory elements within  the Nanog promoter, namely Oct-4 and Sox-2 binding sites, have been identified  to regulate the transcriptional activity of Nanog gene.	bind
31274	2	9102	6	NULL	NULL	0	NULL	Nanog	NULL		regulate	NULL			Sox-2 binding site of promoter	Nanog gene	NULL	transcriptional activity of			NULL		0	NULL	NULL	NULL	abs-batch0620-0649_cell-res_16_3_16541131_s_3	16541131	A 5' flank sequence of the Nanog gene has been  reported to be regulated differentially, and two regulatory elements within  the Nanog promoter, namely Oct-4 and Sox-2 binding sites, have been identified  to regulate the transcriptional activity of Nanog gene.	bind
48004	3	9102	6	10	NULL	0	NULL		NULL		is a type of	NULL			Oct-4 binding site	Nanog	NULL			 regulatory elements within  promoter	NULL		0	NULL	NULL	NULL	abs-batch0620-0649_cell-res_16_3_16541131_s_3	16541131	A 5' flank sequence of the Nanog gene has been  reported to be regulated differentially, and two regulatory elements within  the Nanog promoter, namely Oct-4 and Sox-2 binding sites, have been identified  to regulate the transcriptional activity of Nanog gene.	bind
48005	4	9102	6	10	NULL	0	NULL		NULL		is a type of	NULL			Sox-2 binding site	Nanog	NULL			regulatory elements within  promoter	NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_cell-res_16_3_16541131_s_3	16541131	A 5' flank sequence of the Nanog gene has been  reported to be regulated differentially, and two regulatory elements within  the Nanog promoter, namely Oct-4 and Sox-2 binding sites, have been identified  to regulate the transcriptional activity of Nanog gene.	bind
49161	1	9104	5	13	NULL	NULL	NULL	PDGF-A gene	GP		is activated in				5''-distal enhanceosome	choriocarcinoma cells	Cell				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_oncogene_24_16_15829977_s_1	15829977	A 5''-distal enhanceosome in the PDGF-A gene is activated in choriocarcinoma cells via ligand-independent binding of vitamin D receptor and constitutive jun kinase signaling..	bind
49162	2	9104	5	13	NULL	NULL	NULL	statement 1	Process		occurs via					jun kinase signaling	Process	constitutive \t			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_oncogene_24_16_15829977_s_1	15829977	A 5''-distal enhanceosome in the PDGF-A gene is activated in choriocarcinoma cells via ligand-independent binding of vitamin D receptor and constitutive jun kinase signaling..	bind
49163	3	9104	5	13	NULL	NULL	NULL	vitamin D receptor	GP	binding of	is independent of					ligand	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_oncogene_24_16_15829977_s_1	15829977	A 5''-distal enhanceosome in the PDGF-A gene is activated in choriocarcinoma cells via ligand-independent binding of vitamin D receptor and constitutive jun kinase signaling..	bind
49164	4	9104	5	13	NULL	NULL	NULL	statement 1	Process		occurs via					statement 3	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_oncogene_24_16_15829977_s_1	15829977	A 5''-distal enhanceosome in the PDGF-A gene is activated in choriocarcinoma cells via ligand-independent binding of vitamin D receptor and constitutive jun kinase signaling..	bind
31275	1	9104	6	NULL	NULL	0	NULL	PDGF-A gene	NULL		is activated in	NULL			distal enhanceosome	choriocarcinoma cells	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_oncogene_24_16_15829977_s_1	15829977	A 5''-distal enhanceosome in the PDGF-A gene is activated in choriocarcinoma cells via ligand-independent binding of vitamin D receptor and constitutive jun kinase signaling..	bind
31276	2	9104	6	NULL	NULL	0	NULL	statement 1	NULL		occurs via	NULL				jun kinase signaling	NULL	constitutive			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_oncogene_24_16_15829977_s_1	15829977	A 5''-distal enhanceosome in the PDGF-A gene is activated in choriocarcinoma cells via ligand-independent binding of vitamin D receptor and constitutive jun kinase signaling..	bind
31277	3	9104	6	NULL	NULL	0	NULL	vitamin D receptor	NULL	binding of	is independent of	NULL				ligand	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_oncogene_24_16_15829977_s_1	15829977	A 5''-distal enhanceosome in the PDGF-A gene is activated in choriocarcinoma cells via ligand-independent binding of vitamin D receptor and constitutive jun kinase signaling..	bind
31278	4	9104	6	NULL	NULL	0	NULL	statement 1	NULL		occurs via	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_oncogene_24_16_15829977_s_1	15829977	A 5''-distal enhanceosome in the PDGF-A gene is activated in choriocarcinoma cells via ligand-independent binding of vitamin D receptor and constitutive jun kinase signaling..	bind
39194	1	9105	5	13	NULL	NULL	NULL	GST-PSD fusion protein	GP	recombinant	bind					F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_38_27201_s_278	10480937	A 5-fold molar excess of Ca2+-calmodulin effectively inhibited binding of recombinant GST-PSD fusion protein to F-actin (~85% decrease) (Fig.  6 A).	bind
39195	2	9105	5	13	NULL	NULL	NULL	Ca2+-calmodulin	GP	excess	inhibit		effectively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_38_27201_s_278	10480937	A 5-fold molar excess of Ca2+-calmodulin effectively inhibited binding of recombinant GST-PSD fusion protein to F-actin (~85% decrease) (Fig.  6 A).	bind
31279	1	9105	6	NULL	NULL	0	NULL	GST-PSD fusion protein	NULL	recombinant	bind	NULL				F-actin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_38_27201_s_278	10480937	A 5-fold molar excess of Ca2+-calmodulin effectively inhibited binding of recombinant GST-PSD fusion protein to F-actin (~85% decrease) (Fig.  6 A).	bind
31280	2	9105	6	NULL	NULL	0	NULL	Ca2+-calmodulin	NULL	excess of	inhibits	NULL	effectively			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_38_27201_s_278	10480937	A 5-fold molar excess of Ca2+-calmodulin effectively inhibited binding of recombinant GST-PSD fusion protein to F-actin (~85% decrease) (Fig.  6 A).	bind
39196	1	9108	5	13	NULL	NULL	NULL	PDPs CB1	GP		bind					CD4	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_508_1_67_s_172	11707270	A 50% inhibition of binding of PDPs CB1 and CB8 to CD4 was obtained for 13B8.	bind
39197	2	9108	5	13	NULL	NULL	NULL	PDPs CB8	GP		bind					CD4	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_508_1_67_s_172	11707270	A 50% inhibition of binding of PDPs CB1 and CB8 to CD4 was obtained for 13B8.	bind
48007	3	9108	5	13	NULL	NULL	NULL	13B8	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_508_1_67_s_172	11707270	A 50% inhibition of binding of PDPs CB1 and CB8 to CD4 was obtained for 13B8.	bind
48008	4	9108	5	13	NULL	NULL	NULL	13B8	GP		inhibits					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_508_1_67_s_172	11707270	A 50% inhibition of binding of PDPs CB1 and CB8 to CD4 was obtained for 13B8.	bind
31282	1	9108	6	NULL	NULL	0	NULL	CB1 PDP	NULL		bind	NULL				CD4	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_508_1_67_s_172	11707270	A 50% inhibition of binding of PDPs CB1 and CB8 to CD4 was obtained for 13B8.	bind
31283	2	9108	6	NULL	NULL	0	NULL	CB8 PDP	NULL		bind	NULL				CD4	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_508_1_67_s_172	11707270	A 50% inhibition of binding of PDPs CB1 and CB8 to CD4 was obtained for 13B8.	bind
31284	3	9108	6	NULL	NULL	0	NULL	13B8	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_508_1_67_s_172	11707270	A 50% inhibition of binding of PDPs CB1 and CB8 to CD4 was obtained for 13B8.	bind
31285	4	9108	6	NULL	NULL	0	NULL	13B8	NULL		inhibits	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_508_1_67_s_172	11707270	A 50% inhibition of binding of PDPs CB1 and CB8 to CD4 was obtained for 13B8.	bind
39198	1	9109	5	13	NULL	NULL	NULL	toxaphene	Chemical		inhibit					ouabain	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_toxicol-lett_18_3_6141653_s_9	6141653	A 50% inhibition of ouabain and dopamine binding was obtained  at 150 and 200 microM of toxaphene.	bind
39199	2	9109	5	13	NULL	NULL	NULL	toxaphene	Chemical		inhibit					dopamine	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_toxicol-lett_18_3_6141653_s_9	6141653	A 50% inhibition of ouabain and dopamine binding was obtained  at 150 and 200 microM of toxaphene.	bind
31286	1	9109	6	10	NULL	0	NULL	toxaphene	NULL		inhibits	NULL				dopamine	NULL	binding of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_toxicol-lett_18_3_6141653_s_9	6141653	A 50% inhibition of ouabain and dopamine binding was obtained  at 150 and 200 microM of toxaphene.	bind
31287	2	9109	6	10	NULL	0	NULL	toxaphene	NULL		inhibits	NULL				ouabain	NULL	binding of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_toxicol-lett_18_3_6141653_s_9	6141653	A 50% inhibition of ouabain and dopamine binding was obtained  at 150 and 200 microM of toxaphene.	bind
39200	1	9110	5	13	NULL	NULL	NULL	PNUTS	GP		mediate			50-amino acid domain		PP1	GP	high affinity binding of			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_16_12574161_s_6	12574161	A 50-amino acid domain  in the center of PNUTS mediated both high affinity PP1 binding and inhibition  of PP1 activity.	bind
39201	2	9110	5	13	NULL	NULL	NULL	PNUTS	GP		mediate			50-amino acid domain		PP1 activity	Process	inhibition of			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_16_12574161_s_6	12574161	A 50-amino acid domain  in the center of PNUTS mediated both high affinity PP1 binding and inhibition  of PP1 activity.	bind
31288	1	9110	6	NULL	NULL	0	NULL	PNUTS	NULL		mediates	NULL		50-amino acid domain		PP1	NULL	high affinity binding of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_16_12574161_s_6	12574161	A 50-amino acid domain  in the center of PNUTS mediated both high affinity PP1 binding and inhibition  of PP1 activity.	bind
31289	2	9110	6	NULL	NULL	0	NULL	PNUTS	NULL		mediates	NULL		50-amino acid domain		PP1 activity	NULL	inhibiton of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_16_12574161_s_6	12574161	A 50-amino acid domain  in the center of PNUTS mediated both high affinity PP1 binding and inhibition  of PP1 activity.	bind
39202	1	9112	5	13	NULL	NULL	NULL	BPS domain	GP		is					50-amino acid region between the PH and SH2 domains	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_20_17172_s_21	11278563	A 50-amino acid region between the PH and SH2 domains (BPS domain) contributes to binding of Grb10 and Grb14 to the IR ( 11,  12).	bind
39203	2	9112	5	13	NULL	NULL	NULL	Grb10	GP		bind					IR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_20_17172_s_21	11278563	A 50-amino acid region between the PH and SH2 domains (BPS domain) contributes to binding of Grb10 and Grb14 to the IR ( 11,  12).	bind
39204	3	9112	5	13	NULL	NULL	NULL	Grb14	GP		bind					IR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_20_17172_s_21	11278563	A 50-amino acid region between the PH and SH2 domains (BPS domain) contributes to binding of Grb10 and Grb14 to the IR ( 11,  12).	bind
57765	4	9112	5	13	NULL	NULL	NULL				contributes to			BPS domain		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_20_17172_s_21	11278563	A 50-amino acid region between the PH and SH2 domains (BPS domain) contributes to binding of Grb10 and Grb14 to the IR ( 11,  12).	bind
57766	5	9112	5	13	NULL	NULL	NULL				contribute to			BPS domain		statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_20_17172_s_21	11278563	A 50-amino acid region between the PH and SH2 domains (BPS domain) contributes to binding of Grb10 and Grb14 to the IR ( 11,  12).	bind
31290	1	9112	6	NULL	NULL	0	NULL	Grb10	NULL		bind	NULL				IR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_20_17172_s_21	11278563	A 50-amino acid region between the PH and SH2 domains (BPS domain) contributes to binding of Grb10 and Grb14 to the IR ( 11,  12).	bind
31291	2	9112	6	NULL	NULL	0	NULL	Grb14	NULL		bind	NULL				IR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_20_17172_s_21	11278563	A 50-amino acid region between the PH and SH2 domains (BPS domain) contributes to binding of Grb10 and Grb14 to the IR ( 11,  12).	bind
31292	3	9112	6	NULL	NULL	0	NULL	BPS domain	NULL		is	NULL				50-amino acid region between the PH and SH2 domains	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_20_17172_s_21	11278563	A 50-amino acid region between the PH and SH2 domains (BPS domain) contributes to binding of Grb10 and Grb14 to the IR ( 11,  12).	bind
31293	4	9112	6	NULL	NULL	0	NULL		NULL		contributes to	NULL		BPS domain		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_20_17172_s_21	11278563	A 50-amino acid region between the PH and SH2 domains (BPS domain) contributes to binding of Grb10 and Grb14 to the IR ( 11,  12).	bind
31294	5	9112	6	NULL	NULL	0	NULL		NULL		contributes to	NULL		BPS domain		statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_20_17172_s_21	11278563	A 50-amino acid region between the PH and SH2 domains (BPS domain) contributes to binding of Grb10 and Grb14 to the IR ( 11,  12).	bind
39205	1	9113	5	13	NULL	NULL	NULL	NS1	NucleicAcid		bind					hnRNP A3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_20_18010_s_245	11886857	A 50-fold excess of either A2RE11 or NS1 11-mer eliminated binding of NS1 to hnRNP A3.	bind
39206	2	9113	5	13	NULL	NULL	NULL	A2RE11	NucleicAcid	excess	eliminate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_20_18010_s_245	11886857	A 50-fold excess of either A2RE11 or NS1 11-mer eliminated binding of NS1 to hnRNP A3.	bind
39207	3	9113	5	13	NULL	NULL	NULL	NS1 11-mer	NucleicAcid	excess	eliminate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_20_18010_s_245	11886857	A 50-fold excess of either A2RE11 or NS1 11-mer eliminated binding of NS1 to hnRNP A3.	bind
31295	1	9113	6	NULL	NULL	0	NULL	NS1	NULL		bind	NULL				hnRNP A3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_20_18010_s_245	11886857	A 50-fold excess of either A2RE11 or NS1 11-mer eliminated binding of NS1 to hnRNP A3.	bind
31296	2	9113	6	NULL	NULL	0	NULL	A2RE11	NULL	excess of	eliminates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_20_18010_s_245	11886857	A 50-fold excess of either A2RE11 or NS1 11-mer eliminated binding of NS1 to hnRNP A3.	bind
31297	3	9113	6	10	NULL	0	NULL	NS1 11-mer		excess of	eliminates					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_20_18010_s_245	11886857	A 50-fold excess of either A2RE11 or NS1 11-mer eliminated binding of NS1 to hnRNP A3.	bind
39208	1	9114	5	13	NULL	NULL	NULL	SREBP	GP		bind					DNA	NucleicAcid	labeled			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_32_19938_s_96	9685328	A 50-fold excess of unlabeled homologous competitor fragment displaced SREBP binding to the labeled DNA.	bind
39209	2	9114	5	13	NULL	NULL	NULL	homologous competitor fragment	GP	excess;;unlabeled	bind					DNA	NucleicAcid	labeled			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_32_19938_s_96	9685328	A 50-fold excess of unlabeled homologous competitor fragment displaced SREBP binding to the labeled DNA.	bind
39210	3	9114	5	13	NULL	NULL	NULL	statement 2	Process		displaces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_32_19938_s_96	9685328	A 50-fold excess of unlabeled homologous competitor fragment displaced SREBP binding to the labeled DNA.	bind
31298	1	9114	6	NULL	NULL	0	NULL	SREBP	NULL		bind	NULL				DNA	NULL	labeled			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_32_19938_s_96	9685328	A 50-fold excess of unlabeled homologous competitor fragment displaced SREBP binding to the labeled DNA.	bind
31299	2	9114	6	10	NULL	0	NULL	homologous competitor fragment		unlabeled;; excess of	bind					 DNA		labeled			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_32_19938_s_96	9685328	A 50-fold excess of unlabeled homologous competitor fragment displaced SREBP binding to the labeled DNA.	bind
57767	3	9114	6	10	NULL	0	NULL	statement 2			displaces					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_32_19938_s_96	9685328	A 50-fold excess of unlabeled homologous competitor fragment displaced SREBP binding to the labeled DNA.	bind
42534	1	9118	5	13	NULL	NULL	NULL	516-bp fragment	GP		encompass									DNase I-hypersensitive site	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_32_33398_s_4	15159395	A 516-bp fragment, encompassing a DNase I-hypersensitive site associated with P2 activity that is still retained in adult liver, contains functional HNF1 and HNF6 binding sites and confers full promoter activity in transient transfections.	bind
42535	2	9118	5	13	NULL	NULL	NULL	statement 1	GP		is associated with					P2	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_32_33398_s_4	15159395	A 516-bp fragment, encompassing a DNase I-hypersensitive site associated with P2 activity that is still retained in adult liver, contains functional HNF1 and HNF6 binding sites and confers full promoter activity in transient transfections.	bind
42536	3	9118	5	13	NULL	NULL	NULL	statement 2	Process		is retained in					liver	OrganismPart	adult			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_32_33398_s_4	15159395	A 516-bp fragment, encompassing a DNase I-hypersensitive site associated with P2 activity that is still retained in adult liver, contains functional HNF1 and HNF6 binding sites and confers full promoter activity in transient transfections.	bind
42537	4	9118	5	13	NULL	NULL	NULL	statement 1	GP		contains							functional		HNF1 binding sites	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_32_33398_s_4	15159395	A 516-bp fragment, encompassing a DNase I-hypersensitive site associated with P2 activity that is still retained in adult liver, contains functional HNF1 and HNF6 binding sites and confers full promoter activity in transient transfections.	bind
42538	5	9118	5	13	NULL	NULL	NULL	statement 1	GP		contains							functional		HNF6 binding sites	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_32_33398_s_4	15159395	A 516-bp fragment, encompassing a DNase I-hypersensitive site associated with P2 activity that is still retained in adult liver, contains functional HNF1 and HNF6 binding sites and confers full promoter activity in transient transfections.	bind
42539	6	9118	5	13	NULL	NULL	NULL	statement 1	GP		confer							full activity of		promoter	NULL	transient transfections	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_32_33398_s_4	15159395	A 516-bp fragment, encompassing a DNase I-hypersensitive site associated with P2 activity that is still retained in adult liver, contains functional HNF1 and HNF6 binding sites and confers full promoter activity in transient transfections.	bind
32023	2	9118	6	10	NULL	0	NULL	statement 1			is associated with					P2 		activity of			NULL	adult liver	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_32_33398_s_4	15159395	A 516-bp fragment, encompassing a DNase I-hypersensitive site associated with P2 activity that is still retained in adult liver, contains functional HNF1 and HNF6 binding sites and confers full promoter activity in transient transfections.	bind
32814	4	9118	6	10	NULL	0	NULL	statement 1	NULL		contains	NULL					NULL	functional		HNF-1 binding site	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_32_33398_s_4	15159395	A 516-bp fragment, encompassing a DNase I-hypersensitive site associated with P2 activity that is still retained in adult liver, contains functional HNF1 and HNF6 binding sites and confers full promoter activity in transient transfections.	bind
32815	5	9118	6	10	NULL	0	NULL	statement 1	NULL		contains	NULL					NULL	functional		HNF6 binding site	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_32_33398_s_4	15159395	A 516-bp fragment, encompassing a DNase I-hypersensitive site associated with P2 activity that is still retained in adult liver, contains functional HNF1 and HNF6 binding sites and confers full promoter activity in transient transfections.	bind
48009	1	9118	6	10	NULL	0	NULL	516-bp fragment			encompass									DNase I-hypersensitive site	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_32_33398_s_4	15159395	A 516-bp fragment, encompassing a DNase I-hypersensitive site associated with P2 activity that is still retained in adult liver, contains functional HNF1 and HNF6 binding sites and confers full promoter activity in transient transfections.	bind
48010	3	9118	6	10	NULL	0	NULL	statement 2			is retained in					 liver		adult			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_32_33398_s_4	15159395	A 516-bp fragment, encompassing a DNase I-hypersensitive site associated with P2 activity that is still retained in adult liver, contains functional HNF1 and HNF6 binding sites and confers full promoter activity in transient transfections.	bind
39211	1	9119	5	13	NULL	NULL	NULL	55 kDa protein	GP		bind					U3 snoRNA	NucleicAcid				NULL	CHO cells	NULL	NULL	NULL	NULL	gw60_gene_313_0_17_s_143	12957375	A 55 kDa protein that bound to U3 snoRNA was isolated for the first time by [  Lubben et al., 1993] in CHO cells.	bind
31352	1	9119	6	10	NULL	0	NULL	55 kDa protein 	NULL		bind	NULL				U3 snoRNA	NULL				NULL	CHO cells	NULL	NULL	NULL	NULL	gw60_gene_313_0_17_s_143	12957375	A 55 kDa protein that bound to U3 snoRNA was isolated for the first time by [  Lubben et al., 1993] in CHO cells.	bind
39213	1	9120	5	13	NULL	NULL	NULL	55-60-kDa protein	GP		bind					Ins	GP			PRS	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_2_1099_s_138	11696543	A 55-60-kDa Protein Binds to the Ins-PRS-- The findings that glucose-induced changes in insulin mRNA stability control insulin mRNA contents prompted us to next investigate the mechanisms that regulate insulin mRNA stability.	bind
39214	2	9120	5	13	NULL	NULL	NULL	glucose	NucleicAcid		induce					insulin mRNA	NucleicAcid	changes in stability of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_2_1099_s_138	11696543	A 55-60-kDa Protein Binds to the Ins-PRS-- The findings that glucose-induced changes in insulin mRNA stability control insulin mRNA contents prompted us to next investigate the mechanisms that regulate insulin mRNA stability.	bind
39215	3	9120	5	13	NULL	NULL	NULL	statement 2	Process		controls					insulin mRNA	NucleicAcid	contents of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_2_1099_s_138	11696543	A 55-60-kDa Protein Binds to the Ins-PRS-- The findings that glucose-induced changes in insulin mRNA stability control insulin mRNA contents prompted us to next investigate the mechanisms that regulate insulin mRNA stability.	bind
31353	1	9120	6	10	NULL	0	NULL	55-60-kDa Protein			bind					Ins				PRS	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_2_1099_s_138	11696543	A 55-60-kDa Protein Binds to the Ins-PRS-- The findings that glucose-induced changes in insulin mRNA stability control insulin mRNA contents prompted us to next investigate the mechanisms that regulate insulin mRNA stability.	bind
48011	2	9120	6	10	NULL	0	NULL	glucose	NULL		induce	NULL				insulin mRNA	NULL	changes in stability of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_2_1099_s_138	11696543	A 55-60-kDa Protein Binds to the Ins-PRS-- The findings that glucose-induced changes in insulin mRNA stability control insulin mRNA contents prompted us to next investigate the mechanisms that regulate insulin mRNA stability.	bind
48012	3	9120	6	10	NULL	0	NULL	statement 2	NULL		controls	NULL				insulin mRNA	NULL	contents of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_2_1099_s_138	11696543	A 55-60-kDa Protein Binds to the Ins-PRS-- The findings that glucose-induced changes in insulin mRNA stability control insulin mRNA contents prompted us to next investigate the mechanisms that regulate insulin mRNA stability.	bind
39216	1	9122	5	13	NULL	NULL	NULL	phage A1-10	Organism		bind					OppA-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_1_51_s_145	14679224	A 6 muM concentration of peptide A1-10P inhibited the binding of phage A1-10 to OppA-1 by 91%; the same concentration of the negative control peptide NB-21P did not inhibit the binding of phage A1-10 to OppA-1.	bind
39217	2	9122	5	13	NULL	NULL	NULL	A1-10P peptide	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_1_51_s_145	14679224	A 6 muM concentration of peptide A1-10P inhibited the binding of phage A1-10 to OppA-1 by 91%; the same concentration of the negative control peptide NB-21P did not inhibit the binding of phage A1-10 to OppA-1.	bind
39218	3	9122	5	13	NULL	NULL	NULL	NB-21P peptide	GP		does not inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_1_51_s_145	14679224	A 6 muM concentration of peptide A1-10P inhibited the binding of phage A1-10 to OppA-1 by 91%; the same concentration of the negative control peptide NB-21P did not inhibit the binding of phage A1-10 to OppA-1.	bind
31359	1	9122	6	NULL	NULL	0	NULL	phage A1-10	NULL		bind	NULL				OppA-1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_1_51_s_145	14679224	A 6 muM concentration of peptide A1-10P inhibited the binding of phage A1-10 to OppA-1 by 91%; the same concentration of the negative control peptide NB-21P did not inhibit the binding of phage A1-10 to OppA-1.	bind
31360	2	9122	6	NULL	NULL	0	NULL	A1-10P peptide	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_1_51_s_145	14679224	A 6 muM concentration of peptide A1-10P inhibited the binding of phage A1-10 to OppA-1 by 91%; the same concentration of the negative control peptide NB-21P did not inhibit the binding of phage A1-10 to OppA-1.	bind
31361	3	9122	6	NULL	NULL	0	NULL	NB-21P peptide	NULL		does not inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_1_51_s_145	14679224	A 6 muM concentration of peptide A1-10P inhibited the binding of phage A1-10 to OppA-1 by 91%; the same concentration of the negative control peptide NB-21P did not inhibit the binding of phage A1-10 to OppA-1.	bind
39219	1	9123	5	13	NULL	NULL	NULL	6-mer heparin oligosaccharide	Chemical		bind					PRELP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_52_40695_s_9	11007795	A 6-mer heparin oligosaccharide was the smallest size showing binding to PRELP.	bind
31362	1	9123	6	10	NULL	0	NULL	6-mer heparin oligosaccharide	NULL		bind	NULL				PRELP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_52_40695_s_9	11007795	A 6-mer heparin oligosaccharide was the smallest size showing binding to PRELP.	bind
39220	1	9124	5	13	NULL	NULL	NULL	VSLAFS	GP		is a type of					6-mer peptide	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_37_27398_s_86	16844690	A 6-mer peptide (VSLAFS, the herein identified C9 consensus sequence that binds to CD59) and 8-mer peptide (DVSLAFSE, synthetic peptide shown to bind CD59) were created as objects in ICM ( ) and docked to both the closed and the open refined conformations of CD59, defined by the set of residues within 3  Ang  of the open structure pocket.	bind
39221	2	9124	5	13	NULL	NULL	NULL	VSLAFS	GP		is a type of					C9 consensus sequence	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_37_27398_s_86	16844690	A 6-mer peptide (VSLAFS, the herein identified C9 consensus sequence that binds to CD59) and 8-mer peptide (DVSLAFSE, synthetic peptide shown to bind CD59) were created as objects in ICM ( ) and docked to both the closed and the open refined conformations of CD59, defined by the set of residues within 3  Ang  of the open structure pocket.	bind
39222	3	9124	5	13	NULL	NULL	NULL	VSLAFS	GP		bind					CD59	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_37_27398_s_86	16844690	A 6-mer peptide (VSLAFS, the herein identified C9 consensus sequence that binds to CD59) and 8-mer peptide (DVSLAFSE, synthetic peptide shown to bind CD59) were created as objects in ICM ( ) and docked to both the closed and the open refined conformations of CD59, defined by the set of residues within 3  Ang  of the open structure pocket.	bind
39223	4	9124	5	13	NULL	NULL	NULL	DVSLAFSE	GP		is a type of					8-mer peptide	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_37_27398_s_86	16844690	A 6-mer peptide (VSLAFS, the herein identified C9 consensus sequence that binds to CD59) and 8-mer peptide (DVSLAFSE, synthetic peptide shown to bind CD59) were created as objects in ICM ( ) and docked to both the closed and the open refined conformations of CD59, defined by the set of residues within 3  Ang  of the open structure pocket.	bind
39224	5	9124	5	13	NULL	NULL	NULL	DVSLAFSE	GP		bind					CD59	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_37_27398_s_86	16844690	A 6-mer peptide (VSLAFS, the herein identified C9 consensus sequence that binds to CD59) and 8-mer peptide (DVSLAFSE, synthetic peptide shown to bind CD59) were created as objects in ICM ( ) and docked to both the closed and the open refined conformations of CD59, defined by the set of residues within 3  Ang  of the open structure pocket.	bind
39225	6	9124	5	13	NULL	NULL	NULL	VSLAFS	GP		is docked to					CD59	GP	closed refined conformations of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_37_27398_s_86	16844690	A 6-mer peptide (VSLAFS, the herein identified C9 consensus sequence that binds to CD59) and 8-mer peptide (DVSLAFSE, synthetic peptide shown to bind CD59) were created as objects in ICM ( ) and docked to both the closed and the open refined conformations of CD59, defined by the set of residues within 3  Ang  of the open structure pocket.	bind
39226	7	9124	5	13	NULL	NULL	NULL	DVSLAFSE	GP		is docked to					CD59	GP	open refined conformations of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_37_27398_s_86	16844690	A 6-mer peptide (VSLAFS, the herein identified C9 consensus sequence that binds to CD59) and 8-mer peptide (DVSLAFSE, synthetic peptide shown to bind CD59) were created as objects in ICM ( ) and docked to both the closed and the open refined conformations of CD59, defined by the set of residues within 3  Ang  of the open structure pocket.	bind
48017	8	9124	5	13	NULL	NULL	NULL	DVSLAFSE	GP		is a type of					synthetic peptide	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_37_27398_s_86	16844690	A 6-mer peptide (VSLAFS, the herein identified C9 consensus sequence that binds to CD59) and 8-mer peptide (DVSLAFSE, synthetic peptide shown to bind CD59) were created as objects in ICM ( ) and docked to both the closed and the open refined conformations of CD59, defined by the set of residues within 3  Ang  of the open structure pocket.	bind
32024	2	9124	6	10	NULL	0	NULL	VSLAFS	NULL		is a type of	NULL				C9 consensus sequence	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_37_27398_s_86	16844690	A 6-mer peptide (VSLAFS, the herein identified C9 consensus sequence that binds to CD59) and 8-mer peptide (DVSLAFSE, synthetic peptide shown to bind CD59) were created as objects in ICM ( ) and docked to both the closed and the open refined conformations of CD59, defined by the set of residues within 3  Ang  of the open structure pocket.	bind
32025	3	9124	6	10	NULL	0	NULL	VSLAFS	NULL		bind	NULL				CD59	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_37_27398_s_86	16844690	A 6-mer peptide (VSLAFS, the herein identified C9 consensus sequence that binds to CD59) and 8-mer peptide (DVSLAFSE, synthetic peptide shown to bind CD59) were created as objects in ICM ( ) and docked to both the closed and the open refined conformations of CD59, defined by the set of residues within 3  Ang  of the open structure pocket.	bind
32026	4	9124	6	10	NULL	0	NULL	DVSLAFSE peptide	NULL		bind	NULL				CD59	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_37_27398_s_86	16844690	A 6-mer peptide (VSLAFS, the herein identified C9 consensus sequence that binds to CD59) and 8-mer peptide (DVSLAFSE, synthetic peptide shown to bind CD59) were created as objects in ICM ( ) and docked to both the closed and the open refined conformations of CD59, defined by the set of residues within 3  Ang  of the open structure pocket.	bind
48013	1	9124	6	10	NULL	0	NULL	VSLAFS	NULL		is a type of	NULL				6-mer peptide	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_37_27398_s_86	16844690	A 6-mer peptide (VSLAFS, the herein identified C9 consensus sequence that binds to CD59) and 8-mer peptide (DVSLAFSE, synthetic peptide shown to bind CD59) were created as objects in ICM ( ) and docked to both the closed and the open refined conformations of CD59, defined by the set of residues within 3  Ang  of the open structure pocket.	bind
48014	5	9124	6	10	NULL	0	NULL	DVSLAFSE peptide	NULL		is a type of	NULL				8-mer peptide	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_37_27398_s_86	16844690	A 6-mer peptide (VSLAFS, the herein identified C9 consensus sequence that binds to CD59) and 8-mer peptide (DVSLAFSE, synthetic peptide shown to bind CD59) were created as objects in ICM ( ) and docked to both the closed and the open refined conformations of CD59, defined by the set of residues within 3  Ang  of the open structure pocket.	bind
48015	6	9124	6	10	NULL	0	NULL	VSLAFS	NULL		docked to	NULL				CD59	NULL	closed refined conformations of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_37_27398_s_86	16844690	A 6-mer peptide (VSLAFS, the herein identified C9 consensus sequence that binds to CD59) and 8-mer peptide (DVSLAFSE, synthetic peptide shown to bind CD59) were created as objects in ICM ( ) and docked to both the closed and the open refined conformations of CD59, defined by the set of residues within 3  Ang  of the open structure pocket.	bind
48016	7	9124	6	10	NULL	0	NULL	DVSLAFSE peptide	NULL		docked to	NULL				CD59	NULL	open refined conformations of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_37_27398_s_86	16844690	A 6-mer peptide (VSLAFS, the herein identified C9 consensus sequence that binds to CD59) and 8-mer peptide (DVSLAFSE, synthetic peptide shown to bind CD59) were created as objects in ICM ( ) and docked to both the closed and the open refined conformations of CD59, defined by the set of residues within 3  Ang  of the open structure pocket.	bind
48018	8	9124	6	10	NULL	0	NULL	DVSLAFSE	NULL		is a type of	NULL				synthetic peptide	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_37_27398_s_86	16844690	A 6-mer peptide (VSLAFS, the herein identified C9 consensus sequence that binds to CD59) and 8-mer peptide (DVSLAFSE, synthetic peptide shown to bind CD59) were created as objects in ICM ( ) and docked to both the closed and the open refined conformations of CD59, defined by the set of residues within 3  Ang  of the open structure pocket.	bind
39227	1	9125	5	13	NULL	NULL	NULL	60-kDa protein	GP		is designated as					FIR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_2_331_s_31	10882074	A 60 kDa Protein Designated FIR Binds the Central Domain of FBP	bind
39228	2	9125	5	13	NULL	NULL	NULL	FIR	GP		bind					FBP	GP		central domain		NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_2_331_s_31	10882074	A 60 kDa Protein Designated FIR Binds the Central Domain of FBP	bind
31363	1	9125	6	10	NULL	0	NULL	FIR	NULL		is a type of	NULL				60 kDa protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcell_5_2_331_s_31	10882074	A 60 kDa Protein Designated FIR Binds the Central Domain of FBP	bind
31364	2	9125	6	NULL	NULL	0	NULL	FIR	NULL		bind	NULL				FBP	NULL		central domain		NULL		0	NULL	NULL	NULL	gw60_molcell_5_2_331_s_31	10882074	A 60 kDa Protein Designated FIR Binds the Central Domain of FBP	bind
39229	1	9126	5	13	NULL	NULL	NULL	GDP molecule	Chemical		bind					EF-Tu	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_17_5899_s_66	15317795	A 60-mul prereaction mixture containing 50 mM Tris-HCl (pH 7.5), 10 mM magnesium acetate, 150 mM NH4Cl, 50 mM beta-mercaptoethanol, 60 muM GTP, 0.8 mM phosphoenolpyruvate (Sigma), 2 U of pyruvate kinase (Sigma), and EF-Tu at the concentrations indicated below was incubated on ice for 25 min in order to replace the GDP molecule bound to EF-Tu by GTP.	bind
48022	2	9126	5	13	NULL	NULL	NULL	GTP	Chemical		bind					EF-Tu	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_17_5899_s_66	15317795	A 60-mul prereaction mixture containing 50 mM Tris-HCl (pH 7.5), 10 mM magnesium acetate, 150 mM NH4Cl, 50 mM beta-mercaptoethanol, 60 muM GTP, 0.8 mM phosphoenolpyruvate (Sigma), 2 U of pyruvate kinase (Sigma), and EF-Tu at the concentrations indicated below was incubated on ice for 25 min in order to replace the GDP molecule bound to EF-Tu by GTP.	bind
48023	3	9126	5	13	NULL	NULL	NULL	statement 2	Process		replace					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_17_5899_s_66	15317795	A 60-mul prereaction mixture containing 50 mM Tris-HCl (pH 7.5), 10 mM magnesium acetate, 150 mM NH4Cl, 50 mM beta-mercaptoethanol, 60 muM GTP, 0.8 mM phosphoenolpyruvate (Sigma), 2 U of pyruvate kinase (Sigma), and EF-Tu at the concentrations indicated below was incubated on ice for 25 min in order to replace the GDP molecule bound to EF-Tu by GTP.	bind
32027	1	9126	6	NULL	NULL	0	NULL	GDP	NULL		bind	NULL				EF-Tu	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_17_5899_s_66	15317795	A 60-mul prereaction mixture containing 50 mM Tris-HCl (pH 7.5), 10 mM magnesium acetate, 150 mM NH4Cl, 50 mM beta-mercaptoethanol, 60 muM GTP, 0.8 mM phosphoenolpyruvate (Sigma), 2 U of pyruvate kinase (Sigma), and EF-Tu at the concentrations indicated below was incubated on ice for 25 min in order to replace the GDP molecule bound to EF-Tu by GTP.	bind
32028	2	9126	6	10	NULL	0	NULL	GTP			bind					EF-Tu					NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_17_5899_s_66	15317795	A 60-mul prereaction mixture containing 50 mM Tris-HCl (pH 7.5), 10 mM magnesium acetate, 150 mM NH4Cl, 50 mM beta-mercaptoethanol, 60 muM GTP, 0.8 mM phosphoenolpyruvate (Sigma), 2 U of pyruvate kinase (Sigma), and EF-Tu at the concentrations indicated below was incubated on ice for 25 min in order to replace the GDP molecule bound to EF-Tu by GTP.	bind
32029	3	9126	6	10	NULL	0	NULL	statement 2			replace					statement 1					NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_17_5899_s_66	15317795	A 60-mul prereaction mixture containing 50 mM Tris-HCl (pH 7.5), 10 mM magnesium acetate, 150 mM NH4Cl, 50 mM beta-mercaptoethanol, 60 muM GTP, 0.8 mM phosphoenolpyruvate (Sigma), 2 U of pyruvate kinase (Sigma), and EF-Tu at the concentrations indicated below was incubated on ice for 25 min in order to replace the GDP molecule bound to EF-Tu by GTP.	bind
39230	1	9127	5	13	NULL	NULL	NULL	61 kDa luciferase polypeptide	GP		does not bind					homopolymers	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_21_20_8091_s_201	11588182	A 61 kDa luciferase polypeptide showed no binding to any of the homopolymers, confirming the RNA-binding activity of the Msi2 and Msi1 proteins.	bind
39231	2	9127	5	13	NULL	NULL	NULL	Msi2 protein	GP		bind					RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_21_20_8091_s_201	11588182	A 61 kDa luciferase polypeptide showed no binding to any of the homopolymers, confirming the RNA-binding activity of the Msi2 and Msi1 proteins.	bind
39232	3	9127	5	13	NULL	NULL	NULL	Msi1 protein	GP		bind					RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_21_20_8091_s_201	11588182	A 61 kDa luciferase polypeptide showed no binding to any of the homopolymers, confirming the RNA-binding activity of the Msi2 and Msi1 proteins.	bind
48024	4	9127	5	13	NULL	NULL	NULL	statement 1	Process		confirms					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_21_20_8091_s_201	11588182	A 61 kDa luciferase polypeptide showed no binding to any of the homopolymers, confirming the RNA-binding activity of the Msi2 and Msi1 proteins.	bind
48025	5	9127	5	13	NULL	NULL	NULL	statement 1	Process		confirms					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_21_20_8091_s_201	11588182	A 61 kDa luciferase polypeptide showed no binding to any of the homopolymers, confirming the RNA-binding activity of the Msi2 and Msi1 proteins.	bind
31365	1	9127	6	NULL	NULL	0	NULL	Msi2 protein	NULL		bind	NULL				RNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_20_8091_s_201	11588182	A 61 kDa luciferase polypeptide showed no binding to any of the homopolymers, confirming the RNA-binding activity of the Msi2 and Msi1 proteins.	bind
31366	2	9127	6	NULL	NULL	0	NULL	Msi1 protein	NULL		bind	NULL				RNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_20_8091_s_201	11588182	A 61 kDa luciferase polypeptide showed no binding to any of the homopolymers, confirming the RNA-binding activity of the Msi2 and Msi1 proteins.	bind
31367	3	9127	6	NULL	NULL	0	NULL	61 kDa luciferase polypeptide	NULL		does not bind	NULL				homopolymers	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_20_8091_s_201	11588182	A 61 kDa luciferase polypeptide showed no binding to any of the homopolymers, confirming the RNA-binding activity of the Msi2 and Msi1 proteins.	bind
48026	4	9127	6	10	NULL	0	NULL	statement 3	NULL		confirms	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_20_8091_s_201	11588182	A 61 kDa luciferase polypeptide showed no binding to any of the homopolymers, confirming the RNA-binding activity of the Msi2 and Msi1 proteins.	bind
48027	5	9127	6	10	NULL	0	NULL	statement 3	NULL		confirms	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_20_8091_s_201	11588182	A 61 kDa luciferase polypeptide showed no binding to any of the homopolymers, confirming the RNA-binding activity of the Msi2 and Msi1 proteins.	bind
39233	1	9129	5	13	NULL	NULL	NULL	65-kDa cellular protein	GP		bind					 Riboprobe	NucleicAcid			NRE	NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_1_163_s_93	8990179	A 65-kDa Cellular Protein Binds to an NRE Riboprobe.	bind
31368	1	9129	6	NULL	NULL	0	NULL	65-kDa Cellular Protein	NULL		bind	NULL				riboprobe	NULL			NRE	NULL		0	NULL	NULL	NULL	gw60_pnas_94_1_163_s_93	8990179	A 65-kDa Cellular Protein Binds to an NRE Riboprobe.	bind
42525	1	9131	5	13	NULL	NULL	NULL	Tpardl	GP		contains				predicted promoter					E boxes	NULL		NULL	NULL	NULL	NULL	gw60_genomeres_10_12_1928_s_171	11116088	A 7-kb region comprising both predicted promoters of  Tpardl includes four E boxes (three subtypes of the 5''-CANNGT-3'' consensus), two fork-head transcription factor sites, a cyclic AMP response element binding (CREB) site, and four Sp1 sites near the P4 promoter.	bind
42526	2	9131	5	13	NULL	NULL	NULL	Tpardl	GP		contains				predicted promoter					fork-head transcription factor sites	NULL		NULL	NULL	NULL	NULL	gw60_genomeres_10_12_1928_s_171	11116088	A 7-kb region comprising both predicted promoters of  Tpardl includes four E boxes (three subtypes of the 5''-CANNGT-3'' consensus), two fork-head transcription factor sites, a cyclic AMP response element binding (CREB) site, and four Sp1 sites near the P4 promoter.	bind
42527	3	9131	5	13	NULL	NULL	NULL	Tpardl	GP		contains				predicted promoter					CREB site	NULL		NULL	NULL	NULL	NULL	gw60_genomeres_10_12_1928_s_171	11116088	A 7-kb region comprising both predicted promoters of  Tpardl includes four E boxes (three subtypes of the 5''-CANNGT-3'' consensus), two fork-head transcription factor sites, a cyclic AMP response element binding (CREB) site, and four Sp1 sites near the P4 promoter.	bind
42528	4	9131	5	13	NULL	NULL	NULL	CREB site	GP		is					cyclic AMP response element binding site	GP				NULL		NULL	NULL	NULL	NULL	gw60_genomeres_10_12_1928_s_171	11116088	A 7-kb region comprising both predicted promoters of  Tpardl includes four E boxes (three subtypes of the 5''-CANNGT-3'' consensus), two fork-head transcription factor sites, a cyclic AMP response element binding (CREB) site, and four Sp1 sites near the P4 promoter.	bind
42529	5	9131	5	13	NULL	NULL	NULL	Tpardl	GP		contains				predicted promoter					Sp1 sites	NULL		NULL	NULL	NULL	NULL	gw60_genomeres_10_12_1928_s_171	11116088	A 7-kb region comprising both predicted promoters of  Tpardl includes four E boxes (three subtypes of the 5''-CANNGT-3'' consensus), two fork-head transcription factor sites, a cyclic AMP response element binding (CREB) site, and four Sp1 sites near the P4 promoter.	bind
42533	6	9131	5	10	NULL	0	NULL		NULL		is located near	NULL			Sp1 sites		NULL			P4 promoter	NULL		NULL	NULL	NULL	NULL	gw60_genomeres_10_12_1928_s_171	11116088	A 7-kb region comprising both predicted promoters of  Tpardl includes four E boxes (three subtypes of the 5''-CANNGT-3'' consensus), two fork-head transcription factor sites, a cyclic AMP response element binding (CREB) site, and four Sp1 sites near the P4 promoter.	bind
40388	1	9131	6	NULL	NULL	0	NULL	Tpardl	NULL		contains	NULL			predicted promoter		NULL			E-boxes	NULL		0	NULL	NULL	NULL	gw60_genomeres_10_12_1928_s_171	11116088	A 7-kb region comprising both predicted promoters of  Tpardl includes four E boxes (three subtypes of the 5''-CANNGT-3'' consensus), two fork-head transcription factor sites, a cyclic AMP response element binding (CREB) site, and four Sp1 sites near the P4 promoter.	bind
40389	2	9131	6	NULL	NULL	0	NULL	Tpardl	NULL		includes	NULL			predicted promoter		NULL			fork-head transcription factor sites	NULL		0	NULL	NULL	NULL	gw60_genomeres_10_12_1928_s_171	11116088	A 7-kb region comprising both predicted promoters of  Tpardl includes four E boxes (three subtypes of the 5''-CANNGT-3'' consensus), two fork-head transcription factor sites, a cyclic AMP response element binding (CREB) site, and four Sp1 sites near the P4 promoter.	bind
40390	3	9131	6	NULL	NULL	0	NULL	Tpardl	NULL		contains	NULL			predicted promoter		NULL			CREB site	NULL		0	NULL	NULL	NULL	gw60_genomeres_10_12_1928_s_171	11116088	A 7-kb region comprising both predicted promoters of  Tpardl includes four E boxes (three subtypes of the 5''-CANNGT-3'' consensus), two fork-head transcription factor sites, a cyclic AMP response element binding (CREB) site, and four Sp1 sites near the P4 promoter.	bind
40391	4	9131	6	NULL	NULL	0	NULL	CREB	NULL		is	NULL				cyclic AMP response element binding	NULL				NULL		0	NULL	NULL	NULL	gw60_genomeres_10_12_1928_s_171	11116088	A 7-kb region comprising both predicted promoters of  Tpardl includes four E boxes (three subtypes of the 5''-CANNGT-3'' consensus), two fork-head transcription factor sites, a cyclic AMP response element binding (CREB) site, and four Sp1 sites near the P4 promoter.	bind
40392	5	9131	6	10	NULL	0	NULL		NULL		is present near	NULL			Sp1 site		NULL			P4 promoter	NULL		NULL	NULL	NULL	NULL	gw60_genomeres_10_12_1928_s_171	11116088	A 7-kb region comprising both predicted promoters of  Tpardl includes four E boxes (three subtypes of the 5''-CANNGT-3'' consensus), two fork-head transcription factor sites, a cyclic AMP response element binding (CREB) site, and four Sp1 sites near the P4 promoter.	bind
48101	6	9131	6	10	NULL	0	NULL	Tpardl	NULL		contains	NULL			predicted promoter	statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_genomeres_10_12_1928_s_171	11116088	A 7-kb region comprising both predicted promoters of  Tpardl includes four E boxes (three subtypes of the 5''-CANNGT-3'' consensus), two fork-head transcription factor sites, a cyclic AMP response element binding (CREB) site, and four Sp1 sites near the P4 promoter.	bind
39234	1	9132	5	13	NULL	NULL	NULL	p72fyn-R	GP		bind					TcR/CD3	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_149_1_181_s_423	10747096	A 72-kilodalton fyn related polypeptide (p72fyn-R) binds to the antigen receptor/CD3 (TcR/CD3) complex.	bind
39235	2	9132	5	13	NULL	NULL	NULL	p72fyn-R	GP		is					72-kilodalton fyn related polypeptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_149_1_181_s_423	10747096	A 72-kilodalton fyn related polypeptide (p72fyn-R) binds to the antigen receptor/CD3 (TcR/CD3) complex.	bind
39236	3	9132	5	13	NULL	NULL	NULL	TcR/CD3	GP		is					antigen receptor/CD3 complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_149_1_181_s_423	10747096	A 72-kilodalton fyn related polypeptide (p72fyn-R) binds to the antigen receptor/CD3 (TcR/CD3) complex.	bind
31395	1	9132	6	NULL	NULL	0	NULL	p72fyn-R	NULL		is	NULL				72-kilodalton fyn related polypeptide	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_149_1_181_s_423	10747096	A 72-kilodalton fyn related polypeptide (p72fyn-R) binds to the antigen receptor/CD3 (TcR/CD3) complex.	bind
31396	2	9132	6	NULL	NULL	0	NULL	TcR/CD3 complex	NULL		is	NULL				antigen receptor/CD3 complex	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_149_1_181_s_423	10747096	A 72-kilodalton fyn related polypeptide (p72fyn-R) binds to the antigen receptor/CD3 (TcR/CD3) complex.	bind
31397	3	9132	6	NULL	NULL	0	NULL	p72fyn-R	NULL		bind	NULL				TcR/CD3 complex	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_149_1_181_s_423	10747096	A 72-kilodalton fyn related polypeptide (p72fyn-R) binds to the antigen receptor/CD3 (TcR/CD3) complex.	bind
39237	1	9133	5	13	NULL	NULL	NULL	75 kDa protein	GP		bind									41 nt region	NULL		NULL	NULL	NULL	NULL	gw60_cell_108_4_533_s_179	11909524	A 75 kDa protein has been shown to bind to a 41 nt region, and binding of this protein may be important for localization (see section on structure of elements below).	bind
39238	2	9133	5	13	NULL	NULL	NULL	statement 1	Process		important for		may be			localization	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_108_4_533_s_179	11909524	A 75 kDa protein has been shown to bind to a 41 nt region, and binding of this protein may be important for localization (see section on structure of elements below).	bind
31398	1	9133	6	NULL	NULL	0	NULL	75 kDa protein	NULL		bind	NULL					NULL			41 nt region	NULL		0	NULL	NULL	NULL	gw60_cell_108_4_533_s_179	11909524	A 75 kDa protein has been shown to bind to a 41 nt region, and binding of this protein may be important for localization (see section on structure of elements below).	bind
57768	2	9133	6	10	NULL	0	NULL	statement 1			important for		may be			localization					NULL		0	NULL	NULL	NULL	gw60_cell_108_4_533_s_179	11909524	A 75 kDa protein has been shown to bind to a 41 nt region, and binding of this protein may be important for localization (see section on structure of elements below).	bind
39239	1	9134	5	13	NULL	NULL	NULL	75-kDa brush border protein	GP		bind		directly			horseradish peroxidase-streptavidin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_6_3509_s_197	10816505	A 75-kDa brush border protein bound the horseradish peroxidase-streptavidin directly ( 9) and was stained prominently regardless of membrane treatment.	bind
31409	1	9134	6	NULL	NULL	0	NULL	75-kDa brush border protein	NULL		bind	NULL	directly			horseradish peroxidase-streptavidin	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3509_s_197	10816505	A 75-kDa brush border protein bound the horseradish peroxidase-streptavidin directly ( 9) and was stained prominently regardless of membrane treatment.	bind
48028	1	9135	5	13	NULL	NULL	NULL	anti-mouse Cdc21 antibody	GP		recognize					 86-kDa protein	GP				NULL	whole cell extracts	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_39_24115_s_105	8798650	A 86-kDa protein in whole cell extracts that was recognized with the anti-mouse Cdc21 antibody did not bind with the histone column.	bind
31410	1	9135	6	NULL	NULL	0	NULL	Cdc21 antibody	NULL		recognizes	NULL				86-kDa protein	NULL				NULL	whole-cell extracts	0	NULL	NULL	NULL	gw60_jbiolchem_271_39_24115_s_105	8798650	A 86-kDa protein in whole cell extracts that was recognized with the anti-mouse Cdc21 antibody did not bind with the histone column.	bind
39240	1	9136	5	13	NULL	NULL	NULL	95-kDa protein	GP		corresponds to					STAT5	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_11_6850_s_86	9054369	A 95-kDa band corresponding to STAT5 was tyrosine-phosphorylated in response to EPO (Fig.  2 B,  lane 2) but not SCF (Fig.  2 B,  lane 3), and DNA binding to a STAT5 DNA element was observed only in EPO-treated cells (Fig.  2 C,  lane 2).	bind
39241	2	9136	5	13	NULL	NULL	NULL	EPO	GP		leads to					STAT5	GP	phosphorylation of	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_11_6850_s_86	9054369	A 95-kDa band corresponding to STAT5 was tyrosine-phosphorylated in response to EPO (Fig.  2 B,  lane 2) but not SCF (Fig.  2 B,  lane 3), and DNA binding to a STAT5 DNA element was observed only in EPO-treated cells (Fig.  2 C,  lane 2).	bind
39242	3	9136	5	13	NULL	NULL	NULL	SCF	GP		does not lead to					STAT5	GP	phosphorylation of	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_11_6850_s_86	9054369	A 95-kDa band corresponding to STAT5 was tyrosine-phosphorylated in response to EPO (Fig.  2 B,  lane 2) but not SCF (Fig.  2 B,  lane 3), and DNA binding to a STAT5 DNA element was observed only in EPO-treated cells (Fig.  2 C,  lane 2).	bind
39243	4	9136	5	13	NULL	NULL	NULL	DNA	NucleicAcid		bind					STAT5	GP			DNA element	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_11_6850_s_86	9054369	A 95-kDa band corresponding to STAT5 was tyrosine-phosphorylated in response to EPO (Fig.  2 B,  lane 2) but not SCF (Fig.  2 B,  lane 3), and DNA binding to a STAT5 DNA element was observed only in EPO-treated cells (Fig.  2 C,  lane 2).	bind
39244	5	9136	5	13	NULL	NULL	NULL	statement 4	Process		occurs in		only			EPO-treated cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_11_6850_s_86	9054369	A 95-kDa band corresponding to STAT5 was tyrosine-phosphorylated in response to EPO (Fig.  2 B,  lane 2) but not SCF (Fig.  2 B,  lane 3), and DNA binding to a STAT5 DNA element was observed only in EPO-treated cells (Fig.  2 C,  lane 2).	bind
49193	1	9136	6	NULL	NULL	0	NULL	95-kDa protein	NULL		corresponds to	NULL				STAT5	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_11_6850_s_86	9054369	A 95-kDa band corresponding to STAT5 was tyrosine-phosphorylated in response to EPO (Fig.  2 B,  lane 2) but not SCF (Fig.  2 B,  lane 3), and DNA binding to a STAT5 DNA element was observed only in EPO-treated cells (Fig.  2 C,  lane 2).	bind
49194	2	9136	6	NULL	NULL	0	NULL	STAT5	NULL	phosphorylation of	occurs in response to	NULL		tyrosine		EPO	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_11_6850_s_86	9054369	A 95-kDa band corresponding to STAT5 was tyrosine-phosphorylated in response to EPO (Fig.  2 B,  lane 2) but not SCF (Fig.  2 B,  lane 3), and DNA binding to a STAT5 DNA element was observed only in EPO-treated cells (Fig.  2 C,  lane 2).	bind
49214	3	9136	6	NULL	NULL	0	NULL	STAT5	NULL	phosphorylation of	does not occur in response to	NULL		tyrosine		SCF	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_11_6850_s_86	9054369	A 95-kDa band corresponding to STAT5 was tyrosine-phosphorylated in response to EPO (Fig.  2 B,  lane 2) but not SCF (Fig.  2 B,  lane 3), and DNA binding to a STAT5 DNA element was observed only in EPO-treated cells (Fig.  2 C,  lane 2).	bind
49215	4	9136	6	NULL	NULL	0	NULL	DNA	NULL		bind	NULL				STAT5 	NULL			DNA element	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_11_6850_s_86	9054369	A 95-kDa band corresponding to STAT5 was tyrosine-phosphorylated in response to EPO (Fig.  2 B,  lane 2) but not SCF (Fig.  2 B,  lane 3), and DNA binding to a STAT5 DNA element was observed only in EPO-treated cells (Fig.  2 C,  lane 2).	bind
49216	5	9136	6	NULL	NULL	0	NULL	statement 4	NULL		occurs in presence of	NULL	only			EPO-treated cells	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_11_6850_s_86	9054369	A 95-kDa band corresponding to STAT5 was tyrosine-phosphorylated in response to EPO (Fig.  2 B,  lane 2) but not SCF (Fig.  2 B,  lane 3), and DNA binding to a STAT5 DNA element was observed only in EPO-treated cells (Fig.  2 C,  lane 2).	bind
39245	1	9137	5	13	NULL	NULL	NULL	95-kDa protein	GP	phosphorylated	bind					Grb2	GP		C-terminal SH3 domain		NULL	CDMer cell lysate	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_2_1171_s_179	9891051	A 95-kDa phosphorylated protein was immunoprecipitated by the C-terminal SH3 domain of Grb2 in the CDMer cell lysate (Fig.  4B), and it is likely that it corresponds to the p95 protein binding to the PI 3-kinase (Fig.  4C and D).	bind
39246	2	9137	5	13	NULL	NULL	NULL	p95 protein	GP		bind					PI 3-kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_2_1171_s_179	9891051	A 95-kDa phosphorylated protein was immunoprecipitated by the C-terminal SH3 domain of Grb2 in the CDMer cell lysate (Fig.  4B), and it is likely that it corresponds to the p95 protein binding to the PI 3-kinase (Fig.  4C and D).	bind
57769	3	9137	5	13	NULL	NULL	NULL	95-kDa protein	GP	phosphorylated	corresponds to		may			p95 protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_2_1171_s_179	9891051	A 95-kDa phosphorylated protein was immunoprecipitated by the C-terminal SH3 domain of Grb2 in the CDMer cell lysate (Fig.  4B), and it is likely that it corresponds to the p95 protein binding to the PI 3-kinase (Fig.  4C and D).	bind
31411	1	9137	6	NULL	NULL	0	NULL	95-kDa protein	NULL	phosphorylated	bind	NULL				Grb2	NULL		C-terminal SH3 domain		NULL	CDMer cell lysate	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_2_1171_s_179	9891051	A 95-kDa phosphorylated protein was immunoprecipitated by the C-terminal SH3 domain of Grb2 in the CDMer cell lysate (Fig.  4B), and it is likely that it corresponds to the p95 protein binding to the PI 3-kinase (Fig.  4C and D).	bind
31412	2	9137	6	NULL	NULL	0	NULL	p95 protein	NULL		bind	NULL				PI 3-kinase	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_2_1171_s_179	9891051	A 95-kDa phosphorylated protein was immunoprecipitated by the C-terminal SH3 domain of Grb2 in the CDMer cell lysate (Fig.  4B), and it is likely that it corresponds to the p95 protein binding to the PI 3-kinase (Fig.  4C and D).	bind
57770	3	9137	6	10	NULL	0	NULL	95-kDa protein		phosphorylated	corresponds to		may			p95 protein					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_2_1171_s_179	9891051	A 95-kDa phosphorylated protein was immunoprecipitated by the C-terminal SH3 domain of Grb2 in the CDMer cell lysate (Fig.  4B), and it is likely that it corresponds to the p95 protein binding to the PI 3-kinase (Fig.  4C and D).	bind
39248	1	9138	5	13	NULL	NULL	NULL	insulin receptor	GP		is			beta subunit		95-kDa protein	GP	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_21_12595_s_115	8647870	A 95-kDa tyrosine-phosphorylated protein  (a beta  subunit of insulin receptor) more efficiently bound to  GST-full-length SHPTP2 rather than to GST-SH2 in response to insulin,  although its association with both GST proteins was weaker when  compared with two other major tyrosine-phosphorylated proteins.	bind
39249	2	9138	5	13	NULL	NULL	NULL	insulin receptor	GP		bind			beta subunit		GST-SHPTP2	GP	full-length			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_21_12595_s_115	8647870	A 95-kDa tyrosine-phosphorylated protein  (a beta  subunit of insulin receptor) more efficiently bound to  GST-full-length SHPTP2 rather than to GST-SH2 in response to insulin,  although its association with both GST proteins was weaker when  compared with two other major tyrosine-phosphorylated proteins.	bind
39250	3	9138	5	13	NULL	NULL	NULL	insulin receptor	GP		bind			beta subunit		GST-SH2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_21_12595_s_115	8647870	A 95-kDa tyrosine-phosphorylated protein  (a beta  subunit of insulin receptor) more efficiently bound to  GST-full-length SHPTP2 rather than to GST-SH2 in response to insulin,  although its association with both GST proteins was weaker when  compared with two other major tyrosine-phosphorylated proteins.	bind
39251	4	9138	5	13	NULL	NULL	NULL	statement 2	Process	affinity of	more efficient than					statement 3	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_21_12595_s_115	8647870	A 95-kDa tyrosine-phosphorylated protein  (a beta  subunit of insulin receptor) more efficiently bound to  GST-full-length SHPTP2 rather than to GST-SH2 in response to insulin,  although its association with both GST proteins was weaker when  compared with two other major tyrosine-phosphorylated proteins.	bind
39252	5	9138	5	13	NULL	NULL	NULL	statement 2	Process		in response to					insulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_21_12595_s_115	8647870	A 95-kDa tyrosine-phosphorylated protein  (a beta  subunit of insulin receptor) more efficiently bound to  GST-full-length SHPTP2 rather than to GST-SH2 in response to insulin,  although its association with both GST proteins was weaker when  compared with two other major tyrosine-phosphorylated proteins.	bind
39253	6	9138	5	13	NULL	NULL	NULL	statement 3	Process		in response to					insulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_21_12595_s_115	8647870	A 95-kDa tyrosine-phosphorylated protein  (a beta  subunit of insulin receptor) more efficiently bound to  GST-full-length SHPTP2 rather than to GST-SH2 in response to insulin,  although its association with both GST proteins was weaker when  compared with two other major tyrosine-phosphorylated proteins.	bind
31413	1	9138	6	10	NULL	0	NULL	 insulin receptor	NULL		is 	NULL		beta subunit of		95-kDa protein	NULL	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_21_12595_s_115	8647870	A 95-kDa tyrosine-phosphorylated protein  (a beta  subunit of insulin receptor) more efficiently bound to  GST-full-length SHPTP2 rather than to GST-SH2 in response to insulin,  although its association with both GST proteins was weaker when  compared with two other major tyrosine-phosphorylated proteins.	bind
31414	2	9138	6	10	NULL	0	NULL	 insulin receptor	NULL		bind	NULL		beta subunit of		GST- SHPTP2	NULL	full-length			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_21_12595_s_115	8647870	A 95-kDa tyrosine-phosphorylated protein  (a beta  subunit of insulin receptor) more efficiently bound to  GST-full-length SHPTP2 rather than to GST-SH2 in response to insulin,  although its association with both GST proteins was weaker when  compared with two other major tyrosine-phosphorylated proteins.	bind
31415	3	9138	6	10	NULL	0	NULL	insulin receptor	NULL		bind	NULL		beta subunit of 		GST-SH2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_21_12595_s_115	8647870	A 95-kDa tyrosine-phosphorylated protein  (a beta  subunit of insulin receptor) more efficiently bound to  GST-full-length SHPTP2 rather than to GST-SH2 in response to insulin,  although its association with both GST proteins was weaker when  compared with two other major tyrosine-phosphorylated proteins.	bind
31416	4	9138	6	NULL	NULL	0	NULL	statement 2	NULL		occurs in response to	NULL				insulin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_21_12595_s_115	8647870	A 95-kDa tyrosine-phosphorylated protein  (a beta  subunit of insulin receptor) more efficiently bound to  GST-full-length SHPTP2 rather than to GST-SH2 in response to insulin,  although its association with both GST proteins was weaker when  compared with two other major tyrosine-phosphorylated proteins.	bind
31417	5	9138	6	NULL	NULL	0	NULL	statement 3	NULL		occurs in response to	NULL				insulin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_21_12595_s_115	8647870	A 95-kDa tyrosine-phosphorylated protein  (a beta  subunit of insulin receptor) more efficiently bound to  GST-full-length SHPTP2 rather than to GST-SH2 in response to insulin,  although its association with both GST proteins was weaker when  compared with two other major tyrosine-phosphorylated proteins.	bind
31418	6	9138	6	NULL	NULL	0	NULL	statement 2	NULL	affinity of	is more than	NULL				statement 3	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_21_12595_s_115	8647870	A 95-kDa tyrosine-phosphorylated protein  (a beta  subunit of insulin receptor) more efficiently bound to  GST-full-length SHPTP2 rather than to GST-SH2 in response to insulin,  although its association with both GST proteins was weaker when  compared with two other major tyrosine-phosphorylated proteins.	bind
39254	1	9141	5	13	NULL	NULL	NULL	CRIM1	GP		does not bind					BMP4	GP				NULL	solution	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_36_34181_s_157	12805376	A and   B, CRIM1 does not bind to BMP4 or BMP7 when incubated in solution.	bind
39255	2	9141	5	13	NULL	NULL	NULL	CRIM1	GP		does not bind					BMP7	GP				NULL	solution	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_36_34181_s_157	12805376	A and   B, CRIM1 does not bind to BMP4 or BMP7 when incubated in solution.	bind
39256	3	9141	5	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_36_34181_s_157	12805376	A and   B, CRIM1 does not bind to BMP4 or BMP7 when incubated in solution.	bind
31419	1	9141	6	NULL	NULL	0	NULL	CRIM1	NULL		does not bind	NULL				BMP4	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_36_34181_s_157	12805376	A and   B, CRIM1 does not bind to BMP4 or BMP7 when incubated in solution.	bind
31420	2	9141	6	NULL	NULL	0	NULL	CRIM1	NULL		does not bind	NULL				BMP7	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_36_34181_s_157	12805376	A and   B, CRIM1 does not bind to BMP4 or BMP7 when incubated in solution.	bind
48029	3	9141	6	10	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_36_34181_s_157	12805376	A and   B, CRIM1 does not bind to BMP4 or BMP7 when incubated in solution.	bind
39257	1	9146	5	13	NULL	NULL	NULL	Ub	GP		bind					UBA(1)	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_12_11926_s_151	14707125	a and  b, 1H,15N HSQC of free Ub and Ub bound to UBA(1) and UBA(2).	bind
39258	2	9146	5	13	NULL	NULL	NULL	Ub	GP		bind					UBA(2)	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_12_11926_s_151	14707125	a and  b, 1H,15N HSQC of free Ub and Ub bound to UBA(1) and UBA(2).	bind
31421	1	9146	6	NULL	NULL	0	NULL	Ub	NULL		bind	NULL				UBA(1)	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11926_s_151	14707125	a and  b, 1H,15N HSQC of free Ub and Ub bound to UBA(1) and UBA(2).	bind
31422	2	9146	6	NULL	NULL	0	NULL	Ub	NULL		bind	NULL				UBA(2)	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11926_s_151	14707125	a and  b, 1H,15N HSQC of free Ub and Ub bound to UBA(1) and UBA(2).	bind
39259	1	9147	5	13	NULL	NULL	NULL	UBA(1)	GP		bind					Ub	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_12_11926_s_95	14707125	a and  b, 500 MHz 1H-15N two-dimensional HSQC spectra of UBA(1) and UBA(2) free and bound to Ub.	bind
39260	2	9147	5	13	NULL	NULL	NULL	UBA(2)	GP		bind					Ub	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_12_11926_s_95	14707125	a and  b, 500 MHz 1H-15N two-dimensional HSQC spectra of UBA(1) and UBA(2) free and bound to Ub.	bind
48030	1	9147	6	10	NULL	0	NULL	UBA(1)	NULL		bind	NULL				Ub	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11926_s_95	14707125	a and  b, 500 MHz 1H-15N two-dimensional HSQC spectra of UBA(1) and UBA(2) free and bound to Ub.	bind
48031	2	9147	6	10	NULL	0	NULL	UBA(2)	NULL		bind	NULL				Ub	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11926_s_95	14707125	a and  b, 500 MHz 1H-15N two-dimensional HSQC spectra of UBA(1) and UBA(2) free and bound to Ub.	bind
39261	1	9148	5	13	NULL	NULL	NULL	BAF	GP		bind					H3	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_51_42252_s_215	16203725	A and  B, BAF binds core histone H3 with nanomolar affinity in microtiter assays.	bind
39262	2	9148	5	13	NULL	NULL	NULL	H3	GP		is a type of					core histone	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_51_42252_s_215	16203725	A and  B, BAF binds core histone H3 with nanomolar affinity in microtiter assays.	bind
31424	1	9148	6	10	NULL	0	NULL	BAF			bind					 H3					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_51_42252_s_215	16203725	A and  B, BAF binds core histone H3 with nanomolar affinity in microtiter assays.	bind
57848	2	9148	6	10	NULL	0	NULL	H3			is a type of					core histone					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_42252_s_215	16203725	A and  B, BAF binds core histone H3 with nanomolar affinity in microtiter assays.	bind
39263	1	9149	5	13	NULL	NULL	NULL	Dkk1-AP	GP		bind					LRP6	GP	full-length			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_20_19883_s_72	15778503	A and  B, binding of Dkk1-AP and sclerostin-AP to full-length LRP6, LRP5, or LacZ.	bind
39264	2	9149	5	13	NULL	NULL	NULL	Dkk1-AP	GP		bind					LRP5	GP	full-length			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_20_19883_s_72	15778503	A and  B, binding of Dkk1-AP and sclerostin-AP to full-length LRP6, LRP5, or LacZ.	bind
39265	3	9149	5	13	NULL	NULL	NULL	Dkk1-AP	GP		bind					LacZ	GP	full-length			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_20_19883_s_72	15778503	A and  B, binding of Dkk1-AP and sclerostin-AP to full-length LRP6, LRP5, or LacZ.	bind
39266	4	9149	5	13	NULL	NULL	NULL	sclerostin-AP	GP		bind					LRP6	GP	full-length			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_20_19883_s_72	15778503	A and  B, binding of Dkk1-AP and sclerostin-AP to full-length LRP6, LRP5, or LacZ.	bind
39267	5	9149	5	13	NULL	NULL	NULL	sclerostin-AP	GP		bind					LRP5	GP	full-length			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_20_19883_s_72	15778503	A and  B, binding of Dkk1-AP and sclerostin-AP to full-length LRP6, LRP5, or LacZ.	bind
39268	6	9149	5	13	NULL	NULL	NULL	sclerostin-AP	GP		bind					LacZ	GP	full-length			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_20_19883_s_72	15778503	A and  B, binding of Dkk1-AP and sclerostin-AP to full-length LRP6, LRP5, or LacZ.	bind
31425	1	9149	6	NULL	NULL	0	NULL	Dkk1-AP	NULL		bind	NULL				LRP6	NULL	full length			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_19883_s_72	15778503	A and  B, binding of Dkk1-AP and sclerostin-AP to full-length LRP6, LRP5, or LacZ.	bind
31426	2	9149	6	NULL	NULL	0	NULL	Dkk1-AP	NULL		bind	NULL				LRP5	NULL	full length			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_19883_s_72	15778503	A and  B, binding of Dkk1-AP and sclerostin-AP to full-length LRP6, LRP5, or LacZ.	bind
31427	3	9149	6	NULL	NULL	0	NULL	sclerostin-AP	NULL		bind	NULL				LRP6	NULL	full length			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_19883_s_72	15778503	A and  B, binding of Dkk1-AP and sclerostin-AP to full-length LRP6, LRP5, or LacZ.	bind
31428	4	9149	6	NULL	NULL	0	NULL	sclerostin-AP	NULL		bind	NULL				LRP5	NULL	full length			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_19883_s_72	15778503	A and  B, binding of Dkk1-AP and sclerostin-AP to full-length LRP6, LRP5, or LacZ.	bind
31429	5	9149	6	10	NULL	0	NULL	Dkk1-AP	NULL		bind	NULL				LacZ	NULL	full-length			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_20_19883_s_72	15778503	A and  B, binding of Dkk1-AP and sclerostin-AP to full-length LRP6, LRP5, or LacZ.	bind
31430	6	9149	6	10	NULL	0	NULL	sclerostin-AP	NULL		bind	NULL				LacZ	NULL	full-length			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_20_19883_s_72	15778503	A and  B, binding of Dkk1-AP and sclerostin-AP to full-length LRP6, LRP5, or LacZ.	bind
39269	1	9150	5	13	NULL	NULL	NULL	E2	GP		bind					HSC	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_12_11329_s_199	15611113	A and  B, binding of E2 to HSC was evaluated by a competition assay.	bind
31431	1	9150	6	NULL	NULL	0	NULL	E2	NULL		bind	NULL				HSC	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_12_11329_s_199	15611113	A and  B, binding of E2 to HSC was evaluated by a competition assay.	bind
39270	1	9151	5	13	NULL	NULL	NULL	JIP1b	GP		bind					APP constructs	GP		cytoplasmic domain		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_30_27567_s_85	12023290	A and  B, binding of JIP1b to the APP cytoplasmic domain (APPcyt) constructs  in vitro.	bind
39271	2	9151	5	13	NULL	NULL	NULL	APPcyt	GP		is					APP cytoplasmic domain	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_30_27567_s_85	12023290	A and  B, binding of JIP1b to the APP cytoplasmic domain (APPcyt) constructs  in vitro.	bind
31432	1	9151	6	10	NULL	0	NULL	JIP1b			bind					APP constructs			cytoplasmic domain		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_30_27567_s_85	12023290	A and  B, binding of JIP1b to the APP cytoplasmic domain (APPcyt) constructs  in vitro.	bind
31433	2	9151	6	10	NULL	0	NULL	APPcyt			is					APP cytoplasmic domain					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_30_27567_s_85	12023290	A and  B, binding of JIP1b to the APP cytoplasmic domain (APPcyt) constructs  in vitro.	bind
57849	1	9152	5	13	NULL	NULL	NULL	E-cadherin	GP	mutant	does not bind			E/761		PS1	GP		A431D-E/761		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_43_36007_s_71	16126725	a and  b, cadherin-negative A431D cell lines stably transfected with vector (A431D,  lanes 1 - 3), WT E-cadherin (A431D-E,  lanes 4 - 6), or E-cadherin mutant E/761 unable to bind PS1 (A431D-E/761,  lanes 7 - 9) were transiently transfected with the beta-catenin mutant S33Y.	bind
57850	1	9152	6	10	NULL	0	NULL	E-cadherin 		mutant	does not bind			E/761		PS1			A431D-E/761		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_43_36007_s_71	16126725	a and  b, cadherin-negative A431D cell lines stably transfected with vector (A431D,  lanes 1 - 3), WT E-cadherin (A431D-E,  lanes 4 - 6), or E-cadherin mutant E/761 unable to bind PS1 (A431D-E/761,  lanes 7 - 9) were transiently transfected with the beta-catenin mutant S33Y.	bind
39272	1	9153	5	13	NULL	NULL	NULL	brevican PLD chimera	GP		bind					B28	Cell				NULL	cell surface	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_16_11431_s_93	10196237	A and  B, cell surface binding of brevican PLD chimera to B28	bind
31434	1	9153	6	10	NULL	0	NULL	brevican PLD chimera	NULL		bind	NULL				B28	NULL				NULL	cell surface	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_16_11431_s_93	10196237	A and  B, cell surface binding of brevican PLD chimera to B28	bind
39273	1	9154	5	13	NULL	NULL	NULL	THP-1	GP		bind					Jurkat cells	Cell	necrotic			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_42_35733_s_216	16107330	A and  B, confocal images of simultaneous  red and  green channels, showing binding between THP-1 and necrotic Jurkat cells that precedes ingestion.	bind
39274	2	9154	5	13	NULL	NULL	NULL	statement 1	Process		precedes					ingestion	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_42_35733_s_216	16107330	A and  B, confocal images of simultaneous  red and  green channels, showing binding between THP-1 and necrotic Jurkat cells that precedes ingestion.	bind
31435	1	9154	6	NULL	NULL	0	NULL	THP-1	NULL		bind	NULL				jurkat cells	NULL	necrotic			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_42_35733_s_216	16107330	A and  B, confocal images of simultaneous  red and  green channels, showing binding between THP-1 and necrotic Jurkat cells that precedes ingestion.	bind
31436	2	9154	6	NULL	NULL	0	NULL	statement 1	NULL		precedes	NULL				ingestion	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_42_35733_s_216	16107330	A and  B, confocal images of simultaneous  red and  green channels, showing binding between THP-1 and necrotic Jurkat cells that precedes ingestion.	bind
39275	2	9155	5	13	NULL	NULL	NULL	COPII proteins	GP		bind					statement 1	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_9_7758_s_177	15623526	A and  B, COPII proteins bound to CHO-K1 derived microsomes were sedimented from unbound proteins  through a 0.3 M sucrose cushion and resolved by SDS-PAGE, then transferred to a polyvinylidene difluoride  membrane.	bind
48032	1	9155	5	13	NULL	NULL	NULL	microsomes	CellComponent		derived from					CHO-K1	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_9_7758_s_177	15623526	A and  B, COPII proteins bound to CHO-K1 derived microsomes were sedimented from unbound proteins  through a 0.3 M sucrose cushion and resolved by SDS-PAGE, then transferred to a polyvinylidene difluoride  membrane.	bind
31437	2	9155	6	10	NULL	0	NULL	COPII proteins	NULL		bind	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_9_7758_s_177	15623526	A and  B, COPII proteins bound to CHO-K1 derived microsomes were sedimented from unbound proteins  through a 0.3 M sucrose cushion and resolved by SDS-PAGE, then transferred to a polyvinylidene difluoride  membrane.	bind
48033	1	9155	6	10	NULL	0	NULL	microsomes	NULL		derived from	NULL				CHO-K1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_9_7758_s_177	15623526	A and  B, COPII proteins bound to CHO-K1 derived microsomes were sedimented from unbound proteins  through a 0.3 M sucrose cushion and resolved by SDS-PAGE, then transferred to a polyvinylidene difluoride  membrane.	bind
49155	1	9157	5	13	NULL	NULL	NULL	Stat1	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_2_867_s_109	10625620	A and  B, DNA binding activities of Stat1 and Stat3 in response to IFN-gamma and IL-3.	bind
49156	2	9157	5	13	NULL	NULL	NULL	Stat3	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_2_867_s_109	10625620	A and  B, DNA binding activities of Stat1 and Stat3 in response to IFN-gamma and IL-3.	bind
49541	3	9157	5	13	NULL	NULL	NULL	statement 1	Process		in response to					IFN-gamma	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_2_867_s_109	10625620	A and  B, DNA binding activities of Stat1 and Stat3 in response to IFN-gamma and IL-3.	bind
49542	4	9157	5	13	NULL	NULL	NULL	statement 2	Process		in response to					IFN-gamma	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_2_867_s_109	10625620	A and  B, DNA binding activities of Stat1 and Stat3 in response to IFN-gamma and IL-3.	bind
49543	5	9157	5	13	NULL	NULL	NULL	statement 1	Process		in response to					IL-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_2_867_s_109	10625620	A and  B, DNA binding activities of Stat1 and Stat3 in response to IFN-gamma and IL-3.	bind
49544	6	9157	5	13	NULL	NULL	NULL	statement 2	Process		in response to					IL-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_2_867_s_109	10625620	A and  B, DNA binding activities of Stat1 and Stat3 in response to IFN-gamma and IL-3.	bind
31438	1	9157	6	NULL	NULL	0	NULL	Stat1	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_2_867_s_109	10625620	A and  B, DNA binding activities of Stat1 and Stat3 in response to IFN-gamma and IL-3.	bind
31439	2	9157	6	NULL	NULL	0	NULL	Stat3	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_2_867_s_109	10625620	A and  B, DNA binding activities of Stat1 and Stat3 in response to IFN-gamma and IL-3.	bind
48034	3	9157	6	10	NULL	0	NULL	statement 1	NULL		in response to	NULL				IFN-gamma	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_2_867_s_109	10625620	A and  B, DNA binding activities of Stat1 and Stat3 in response to IFN-gamma and IL-3.	bind
48035	4	9157	6	10	NULL	0	NULL	statement 2	NULL		in response to	NULL				 IL-3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_2_867_s_109	10625620	A and  B, DNA binding activities of Stat1 and Stat3 in response to IFN-gamma and IL-3.	bind
49554	5	9157	6	10	NULL	0	NULL	statement 1	NULL		in response to	NULL				IL-3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_2_867_s_109	10625620	A and  B, DNA binding activities of Stat1 and Stat3 in response to IFN-gamma and IL-3.	bind
49555	6	9157	6	10	NULL	0	NULL	statement 2	NULL		in response to	NULL				IFN-gamma	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_2_867_s_109	10625620	A and  B, DNA binding activities of Stat1 and Stat3 in response to IFN-gamma and IL-3.	bind
39529	1	9159	5	13	NULL	NULL	NULL	GlnR	GP		bind					glnR	GP			(P glnR-1) promoter region	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_35_25097_s_260	16787930	A and  B, EMSA of binding of GlnR to the  glnR (P glnR-1) and  glnP (P glnP-1) promoter regions and to truncated  glnR (P glnR-2) and  glnP (P glnP-2) promoters, lacking their respective GlnR operators.	bind
39530	2	9159	5	13	NULL	NULL	NULL	GlnR	GP		bind					glnP	GP			(P glnP-1) promoter region	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_35_25097_s_260	16787930	A and  B, EMSA of binding of GlnR to the  glnR (P glnR-1) and  glnP (P glnP-1) promoter regions and to truncated  glnR (P glnR-2) and  glnP (P glnP-2) promoters, lacking their respective GlnR operators.	bind
39531	3	9159	5	13	NULL	NULL	NULL	glnR	GP	truncated	lacks				(P glnR-2) promoter	GlnR	GP	respective		operators	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_35_25097_s_260	16787930	A and  B, EMSA of binding of GlnR to the  glnR (P glnR-1) and  glnP (P glnP-1) promoter regions and to truncated  glnR (P glnR-2) and  glnP (P glnP-2) promoters, lacking their respective GlnR operators.	bind
39532	4	9159	5	13	NULL	NULL	NULL	glnP	GP	truncated	lacks				(P glnP-2) promoter	GlnR	GP	respective		operators	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_35_25097_s_260	16787930	A and  B, EMSA of binding of GlnR to the  glnR (P glnR-1) and  glnP (P glnP-1) promoter regions and to truncated  glnR (P glnR-2) and  glnP (P glnP-2) promoters, lacking their respective GlnR operators.	bind
39533	5	9159	5	13	NULL	NULL	NULL	GlnR	GP		bind					statement 3	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_35_25097_s_260	16787930	A and  B, EMSA of binding of GlnR to the  glnR (P glnR-1) and  glnP (P glnP-1) promoter regions and to truncated  glnR (P glnR-2) and  glnP (P glnP-2) promoters, lacking their respective GlnR operators.	bind
39534	6	9159	5	13	NULL	NULL	NULL	GlnR	GP		bind					statement 4	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_35_25097_s_260	16787930	A and  B, EMSA of binding of GlnR to the  glnR (P glnR-1) and  glnP (P glnP-1) promoter regions and to truncated  glnR (P glnR-2) and  glnP (P glnP-2) promoters, lacking their respective GlnR operators.	bind
31440	1	9159	6	NULL	NULL	0	NULL	GlnR	NULL		bind	NULL				glnR	NULL			P glnR-1 site on promoter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_35_25097_s_260	16787930	A and  B, EMSA of binding of GlnR to the  glnR (P glnR-1) and  glnP (P glnP-1) promoter regions and to truncated  glnR (P glnR-2) and  glnP (P glnP-2) promoters, lacking their respective GlnR operators.	bind
31444	2	9159	6	NULL	NULL	0	NULL	GlnR	NULL		bind	NULL				glnP	NULL			P glnP-1 site on promoter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_35_25097_s_260	16787930	A and  B, EMSA of binding of GlnR to the  glnR (P glnR-1) and  glnP (P glnP-1) promoter regions and to truncated  glnR (P glnR-2) and  glnP (P glnP-2) promoters, lacking their respective GlnR operators.	bind
31445	3	9159	6	NULL	NULL	0	NULL	GlnR	NULL		bind	NULL				glnR	NULL	truncated		P glnR-2 site on promoter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_35_25097_s_260	16787930	A and  B, EMSA of binding of GlnR to the  glnR (P glnR-1) and  glnP (P glnP-1) promoter regions and to truncated  glnR (P glnR-2) and  glnP (P glnP-2) promoters, lacking their respective GlnR operators.	bind
31446	4	9159	6	NULL	NULL	0	NULL	GlnR	NULL		bind	NULL				glnP	NULL	truncated		P glnP-2 site on promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_35_25097_s_260	16787930	A and  B, EMSA of binding of GlnR to the  glnR (P glnR-1) and  glnP (P glnP-1) promoter regions and to truncated  glnR (P glnR-2) and  glnP (P glnP-2) promoters, lacking their respective GlnR operators.	bind
48036	5	9159	6	10	NULL	0	NULL	glnR	NULL	truncated	lack	NULL			P glnR-2 site in promoter	glnR	NULL			operator	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_35_25097_s_260	16787930	A and  B, EMSA of binding of GlnR to the  glnR (P glnR-1) and  glnP (P glnP-1) promoter regions and to truncated  glnR (P glnR-2) and  glnP (P glnP-2) promoters, lacking their respective GlnR operators.	bind
48037	6	9159	6	10	NULL	0	NULL	glnP	NULL	truncated	lack	NULL			P glnP-2 site in promoter	glnP	NULL			operator	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_35_25097_s_260	16787930	A and  B, EMSA of binding of GlnR to the  glnR (P glnR-1) and  glnP (P glnP-1) promoter regions and to truncated  glnR (P glnR-2) and  glnP (P glnP-2) promoters, lacking their respective GlnR operators.	bind
39276	1	9160	5	13	NULL	NULL	NULL	FBP30	GP		bind			WW-A domain		PPR-based peptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_14_10359_s_234	10744724	A and  B, fluorescence polarization anisotropy measurements demonstrate that the FBP30 WW-A domain binds a PPR-based peptide, but not a PP XY peptide, in contrast to YAP which binds a PP XY peptide, but not a PPR-based peptide.	bind
39277	2	9160	5	13	NULL	NULL	NULL	FBP30	GP		does not bind			WW-A domain		PP XY peptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_14_10359_s_234	10744724	A and  B, fluorescence polarization anisotropy measurements demonstrate that the FBP30 WW-A domain binds a PPR-based peptide, but not a PP XY peptide, in contrast to YAP which binds a PP XY peptide, but not a PPR-based peptide.	bind
39278	3	9160	5	13	NULL	NULL	NULL	YAP	GP		bind					PP XY peptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_14_10359_s_234	10744724	A and  B, fluorescence polarization anisotropy measurements demonstrate that the FBP30 WW-A domain binds a PPR-based peptide, but not a PP XY peptide, in contrast to YAP which binds a PP XY peptide, but not a PPR-based peptide.	bind
39279	4	9160	5	13	NULL	NULL	NULL	YAP	GP		does not bind					PPR-based peptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_14_10359_s_234	10744724	A and  B, fluorescence polarization anisotropy measurements demonstrate that the FBP30 WW-A domain binds a PPR-based peptide, but not a PP XY peptide, in contrast to YAP which binds a PP XY peptide, but not a PPR-based peptide.	bind
31447	1	9160	6	NULL	NULL	0	NULL	FBP30	NULL		bind	NULL		WW-A domain		PPR-based peptide	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_14_10359_s_234	10744724	A and  B, fluorescence polarization anisotropy measurements demonstrate that the FBP30 WW-A domain binds a PPR-based peptide, but not a PP XY peptide, in contrast to YAP which binds a PP XY peptide, but not a PPR-based peptide.	bind
31448	2	9160	6	NULL	NULL	0	NULL	FBP30	NULL		does not bind	NULL		WW-A domain		PP XY peptide	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_14_10359_s_234	10744724	A and  B, fluorescence polarization anisotropy measurements demonstrate that the FBP30 WW-A domain binds a PPR-based peptide, but not a PP XY peptide, in contrast to YAP which binds a PP XY peptide, but not a PPR-based peptide.	bind
31449	3	9160	6	NULL	NULL	0	NULL	YAP	NULL		bind	NULL				PP XY peptide	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_14_10359_s_234	10744724	A and  B, fluorescence polarization anisotropy measurements demonstrate that the FBP30 WW-A domain binds a PPR-based peptide, but not a PP XY peptide, in contrast to YAP which binds a PP XY peptide, but not a PPR-based peptide.	bind
31450	4	9160	6	NULL	NULL	0	NULL	YAP	NULL		does not bind	NULL				PPR-based peptide	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_14_10359_s_234	10744724	A and  B, fluorescence polarization anisotropy measurements demonstrate that the FBP30 WW-A domain binds a PPR-based peptide, but not a PP XY peptide, in contrast to YAP which binds a PP XY peptide, but not a PPR-based peptide.	bind
39280	1	9161	5	13	NULL	NULL	NULL	SMAD3	GP		does not bind					apoCIII	GP	proximal		HRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_52_41405_s_148	10995777	A and  B, gel electrophoretic mobility shift assays showing that SMAD3 cannot bind to the proximal apoCIII  HRE.	bind
31451	1	9161	6	NULL	NULL	0	NULL	SMAD3	NULL		does not bind	NULL				apoCIII	NULL	proximal		HRE 	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_52_41405_s_148	10995777	A and  B, gel electrophoretic mobility shift assays showing that SMAD3 cannot bind to the proximal apoCIII  HRE.	bind
39281	1	9162	5	13	NULL	NULL	NULL	rSp1	GP		bind					Sp1-A oligos	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_39_40451_s_262	15265862	A and  B, gel shift assay of rSp1 binding to Sp1-A and Sp1-B oligos.	bind
39282	2	9162	5	13	NULL	NULL	NULL	rSp1	GP		bind					Sp1-B oligos	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_39_40451_s_262	15265862	A and  B, gel shift assay of rSp1 binding to Sp1-A and Sp1-B oligos.	bind
31452	1	9162	6	10	NULL	0	NULL	rSp1			bind					Sp1-A oligos					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_39_40451_s_262	15265862	A and  B, gel shift assay of rSp1 binding to Sp1-A and Sp1-B oligos.	bind
31453	2	9162	6	10	NULL	0	NULL	rSp1			bind					Sp1-B oligos					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_39_40451_s_262	15265862	A and  B, gel shift assay of rSp1 binding to Sp1-A and Sp1-B oligos.	bind
39283	1	9165	5	13	NULL	NULL	NULL	GAR	GP		bind					histones	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_49_50930_s_185	15456770	A and  B, in vitro binding of GAR and histones.	bind
31454	1	9165	6	10	NULL	0	NULL	GAR			bind					histones					NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_49_50930_s_185	15456770	A and  B, in vitro binding of GAR and histones.	bind
39284	1	9166	5	13	NULL	NULL	NULL	ERK1/2	GP		bind					MEK1	GP		KIM-SL		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_45_37885_s_251	16148006	A and  B, increased binding of ERK1/2 to (KIM-SL)MEK1.	bind
31455	1	9166	6	NULL	NULL	0	NULL	ERK1/2	NULL		bind	NULL				MEK1	NULL		KIM-SL		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_45_37885_s_251	16148006	A and  B, increased binding of ERK1/2 to (KIM-SL)MEK1.	bind
39285	1	9168	5	13	NULL	NULL	NULL	MEKK2	GP		bind					PRK2	GP		residues 479-670		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24421_s_104	10818102	A and  B, MEKK2 binds PRK2 (residues 479-670) in the yeast two-hybrid system.	bind
31456	1	9168	6	NULL	NULL	0	NULL	MEKK2	NULL		bind	NULL				PRK2	NULL		479-670		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24421_s_104	10818102	A and  B, MEKK2 binds PRK2 (residues 479-670) in the yeast two-hybrid system.	bind
39286	1	9169	5	13	NULL	NULL	NULL	MyD88	GP		is required for					TLR8 	GP	signaling of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_21013_s_137	16737960	a and  b, MyD88 and IRAK are required for TLR8 signaling.	bind
39287	2	9169	5	13	NULL	NULL	NULL	IRAK	GP		is required for					TLR8 	GP	signaling of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_21013_s_137	16737960	a and  b, MyD88 and IRAK are required for TLR8 signaling.	bind
31457	1	9169	6	NULL	NULL	0	NULL	MyD88	NULL		is required for	NULL				TLR8	NULL	signaling of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21013_s_137	16737960	a and  b, MyD88 and IRAK are required for TLR8 signaling.	bind
31458	2	9169	6	NULL	NULL	0	NULL	IRAK	NULL		is required for	NULL				TLR8	NULL	signaling of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21013_s_137	16737960	a and  b, MyD88 and IRAK are required for TLR8 signaling.	bind
39535	1	9171	5	13	NULL	NULL	NULL	Rab11a	GP		bind					GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_32_33430_s_133	15173169	A and  B, Rip11-F1 titration with the GDP- and Gpp(NH)p-bound forms of Rab11a, respectively;   C and  D, Rip11-F1 titration with the GDP- and Gpp(NH)p-bound forms of Rab11b, respectively;   E and  F, buffer titration with the GDP- and Gpp(NH)p-bound forms of Rab11a, respectively.	bind
39536	2	9171	5	13	NULL	NULL	NULL	Rab11a	GP		bind					Gpp(NH)p	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_32_33430_s_133	15173169	A and  B, Rip11-F1 titration with the GDP- and Gpp(NH)p-bound forms of Rab11a, respectively;   C and  D, Rip11-F1 titration with the GDP- and Gpp(NH)p-bound forms of Rab11b, respectively;   E and  F, buffer titration with the GDP- and Gpp(NH)p-bound forms of Rab11a, respectively.	bind
39537	3	9171	5	13	NULL	NULL	NULL	Rab11b	GP		bind					GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_32_33430_s_133	15173169	A and  B, Rip11-F1 titration with the GDP- and Gpp(NH)p-bound forms of Rab11a, respectively;   C and  D, Rip11-F1 titration with the GDP- and Gpp(NH)p-bound forms of Rab11b, respectively;   E and  F, buffer titration with the GDP- and Gpp(NH)p-bound forms of Rab11a, respectively.	bind
39538	4	9171	5	13	NULL	NULL	NULL	Rab11b	GP		bind					Gpp(NH)p	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_32_33430_s_133	15173169	A and  B, Rip11-F1 titration with the GDP- and Gpp(NH)p-bound forms of Rab11a, respectively;   C and  D, Rip11-F1 titration with the GDP- and Gpp(NH)p-bound forms of Rab11b, respectively;   E and  F, buffer titration with the GDP- and Gpp(NH)p-bound forms of Rab11a, respectively.	bind
31545	1	9171	6	NULL	NULL	0	NULL	GDP	NULL		bind	NULL				Rab11a	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_32_33430_s_133	15173169	A and  B, Rip11-F1 titration with the GDP- and Gpp(NH)p-bound forms of Rab11a, respectively;   C and  D, Rip11-F1 titration with the GDP- and Gpp(NH)p-bound forms of Rab11b, respectively;   E and  F, buffer titration with the GDP- and Gpp(NH)p-bound forms of Rab11a, respectively.	bind
31546	2	9171	6	NULL	NULL	0	NULL	Gpp(NH)p	NULL		bind	NULL				Rab11a	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_32_33430_s_133	15173169	A and  B, Rip11-F1 titration with the GDP- and Gpp(NH)p-bound forms of Rab11a, respectively;   C and  D, Rip11-F1 titration with the GDP- and Gpp(NH)p-bound forms of Rab11b, respectively;   E and  F, buffer titration with the GDP- and Gpp(NH)p-bound forms of Rab11a, respectively.	bind
31547	3	9171	6	NULL	NULL	0	NULL	GDP	NULL		bind	NULL				Rab11b	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_32_33430_s_133	15173169	A and  B, Rip11-F1 titration with the GDP- and Gpp(NH)p-bound forms of Rab11a, respectively;   C and  D, Rip11-F1 titration with the GDP- and Gpp(NH)p-bound forms of Rab11b, respectively;   E and  F, buffer titration with the GDP- and Gpp(NH)p-bound forms of Rab11a, respectively.	bind
31548	4	9171	6	NULL	NULL	0	NULL	Gpp(NH)p	NULL		bind	NULL				Rab11b	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_32_33430_s_133	15173169	A and  B, Rip11-F1 titration with the GDP- and Gpp(NH)p-bound forms of Rab11a, respectively;   C and  D, Rip11-F1 titration with the GDP- and Gpp(NH)p-bound forms of Rab11b, respectively;   E and  F, buffer titration with the GDP- and Gpp(NH)p-bound forms of Rab11a, respectively.	bind
39288	1	9172	5	13	NULL	NULL	NULL	C2AB	GP		bind					PS/PtdIns(4, 5)P2-containing vesicles	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_17_10240_s_205	9553075	A and  B, Rp(676-695) specifically inhibits binding of C2AB to PS/PtdIns(4, 5)P2-containing vesicles,  C, a related peptide directly binds lipid vesicles.	bind
39289	2	9172	5	13	NULL	NULL	NULL	Rp	GP		inhibit		specifically	676-695		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_17_10240_s_205	9553075	A and  B, Rp(676-695) specifically inhibits binding of C2AB to PS/PtdIns(4, 5)P2-containing vesicles,  C, a related peptide directly binds lipid vesicles.	bind
39290	3	9172	5	13	NULL	NULL	NULL	peptide related to Rp	GP		bind		directly	676-695		lipid vesicles	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_17_10240_s_205	9553075	A and  B, Rp(676-695) specifically inhibits binding of C2AB to PS/PtdIns(4, 5)P2-containing vesicles,  C, a related peptide directly binds lipid vesicles.	bind
31803	1	9172	6	NULL	NULL	0	NULL	C2AB	NULL		bind	NULL				PS/PtdIns(4, 5)P2-containing vesicles	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_17_10240_s_205	9553075	A and  B, Rp(676-695) specifically inhibits binding of C2AB to PS/PtdIns(4, 5)P2-containing vesicles,  C, a related peptide directly binds lipid vesicles.	bind
31804	2	9172	6	NULL	NULL	0	NULL	Rp	NULL		inhibits	NULL	specifically	676-695		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_17_10240_s_205	9553075	A and  B, Rp(676-695) specifically inhibits binding of C2AB to PS/PtdIns(4, 5)P2-containing vesicles,  C, a related peptide directly binds lipid vesicles.	bind
31805	3	9172	6	10	NULL	0	NULL	peptide related to Rp	NULL		bind	NULL	directly	676-695		lipid vesicles	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_17_10240_s_205	9553075	A and  B, Rp(676-695) specifically inhibits binding of C2AB to PS/PtdIns(4, 5)P2-containing vesicles,  C, a related peptide directly binds lipid vesicles.	bind
48038	1	9173	5	13	NULL	NULL	NULL	tau	GP		does not bind					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_9_7614_s_168	15611092	A and  B, SDS-PAGE of free (tau not bound to heparin) and bound (tau bound to heparin) tau  following incubation with heparin-Sepharose in the absence ( Con.) or the presence of inhibitory compounds (exifone, methylene blue, and hematin).	bind
48039	2	9173	5	13	NULL	NULL	NULL	tau	GP		bind					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_9_7614_s_168	15611092	A and  B, SDS-PAGE of free (tau not bound to heparin) and bound (tau bound to heparin) tau  following incubation with heparin-Sepharose in the absence ( Con.) or the presence of inhibitory compounds (exifone, methylene blue, and hematin).	bind
31806	1	9173	6	NULL	NULL	0	NULL	tau	NULL		does not bind	NULL				heparin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_9_7614_s_168	15611092	A and  B, SDS-PAGE of free (tau not bound to heparin) and bound (tau bound to heparin) tau  following incubation with heparin-Sepharose in the absence ( Con.) or the presence of inhibitory compounds (exifone, methylene blue, and hematin).	bind
31807	2	9173	6	NULL	NULL	0	NULL	tau	NULL		bind	NULL				heparin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_9_7614_s_168	15611092	A and  B, SDS-PAGE of free (tau not bound to heparin) and bound (tau bound to heparin) tau  following incubation with heparin-Sepharose in the absence ( Con.) or the presence of inhibitory compounds (exifone, methylene blue, and hematin).	bind
39291	1	9174	5	13	NULL	NULL	NULL	CLOCK-BMAL1 heterodimer	GP		bind									E-box	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_51_42036_s_288	16249183	A and  B, shown are the transcription mechanisms of binding of the CLOCK-BMAL1 heterodimer  to the E-box for the rhythmic expression of  Per1 and of binding of CREB to the CRE for transient expression of  Per1, respectively.	bind
39292	2	9174	5	13	NULL	NULL	NULL	statement 1	Process		is required for					Per1	GP	rhythmic expression of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_51_42036_s_288	16249183	A and  B, shown are the transcription mechanisms of binding of the CLOCK-BMAL1 heterodimer  to the E-box for the rhythmic expression of  Per1 and of binding of CREB to the CRE for transient expression of  Per1, respectively.	bind
39293	3	9174	5	13	NULL	NULL	NULL	CREB	GP		bind									CRE	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_51_42036_s_288	16249183	A and  B, shown are the transcription mechanisms of binding of the CLOCK-BMAL1 heterodimer  to the E-box for the rhythmic expression of  Per1 and of binding of CREB to the CRE for transient expression of  Per1, respectively.	bind
39294	4	9174	5	13	NULL	NULL	NULL	statement 3	Process		is required for					Per1	GP	transient expression of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_51_42036_s_288	16249183	A and  B, shown are the transcription mechanisms of binding of the CLOCK-BMAL1 heterodimer  to the E-box for the rhythmic expression of  Per1 and of binding of CREB to the CRE for transient expression of  Per1, respectively.	bind
31808	1	9174	6	NULL	NULL	0	NULL	CLOCK-BMAL1 heterodimer	NULL		bind	NULL					NULL			E box	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_42036_s_288	16249183	A and  B, shown are the transcription mechanisms of binding of the CLOCK-BMAL1 heterodimer  to the E-box for the rhythmic expression of  Per1 and of binding of CREB to the CRE for transient expression of  Per1, respectively.	bind
31809	2	9174	6	NULL	NULL	0	NULL	statement 1	NULL		is required for	NULL				Per1	NULL	rhythmic expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_42036_s_288	16249183	A and  B, shown are the transcription mechanisms of binding of the CLOCK-BMAL1 heterodimer  to the E-box for the rhythmic expression of  Per1 and of binding of CREB to the CRE for transient expression of  Per1, respectively.	bind
31810	3	9174	6	NULL	NULL	0	NULL	CREB	NULL		bind	NULL					NULL			CRE	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_42036_s_288	16249183	A and  B, shown are the transcription mechanisms of binding of the CLOCK-BMAL1 heterodimer  to the E-box for the rhythmic expression of  Per1 and of binding of CREB to the CRE for transient expression of  Per1, respectively.	bind
31811	4	9174	6	NULL	NULL	0	NULL	statement 3	NULL		is required for	NULL				Per1	NULL	transient expression of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_42036_s_288	16249183	A and  B, shown are the transcription mechanisms of binding of the CLOCK-BMAL1 heterodimer  to the E-box for the rhythmic expression of  Per1 and of binding of CREB to the CRE for transient expression of  Per1, respectively.	bind
39295	1	9175	5	13	NULL	NULL	NULL	Sp1	GP		bind			ZFDBD		SMRT	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_30_28061_s_305	15878880	A and  B, Sp1ZFDBD is bound by the corepressors SMRT and NCoR, and has no access to the target  Sp1-binding GC boxes in the promoters or the enhancers.	bind
39296	2	9175	5	13	NULL	NULL	NULL	Sp1	GP		bind			ZFDBD		NCoR	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_30_28061_s_305	15878880	A and  B, Sp1ZFDBD is bound by the corepressors SMRT and NCoR, and has no access to the target  Sp1-binding GC boxes in the promoters or the enhancers.	bind
39297	3	9175	5	13	NULL	NULL	NULL	NCoR	GP		is a type of					corepressor	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_30_28061_s_305	15878880	A and  B, Sp1ZFDBD is bound by the corepressors SMRT and NCoR, and has no access to the target  Sp1-binding GC boxes in the promoters or the enhancers.	bind
39298	4	9175	5	13	NULL	NULL	NULL	SMRT	GP		is a type of					corepressor	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_30_28061_s_305	15878880	A and  B, Sp1ZFDBD is bound by the corepressors SMRT and NCoR, and has no access to the target  Sp1-binding GC boxes in the promoters or the enhancers.	bind
39299	7	9175	5	13	NULL	NULL	NULL	statement 1	GP		does not have access to					statement 5	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_30_28061_s_305	15878880	A and  B, Sp1ZFDBD is bound by the corepressors SMRT and NCoR, and has no access to the target  Sp1-binding GC boxes in the promoters or the enhancers.	bind
39300	8	9175	5	13	NULL	NULL	NULL	statement 1	GP		does not have access to					statement 6	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_30_28061_s_305	15878880	A and  B, Sp1ZFDBD is bound by the corepressors SMRT and NCoR, and has no access to the target  Sp1-binding GC boxes in the promoters or the enhancers.	bind
39302	9	9175	5	13	NULL	NULL	NULL	statement 2	GP		does not have access to					statement 5	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_30_28061_s_305	15878880	A and  B, Sp1ZFDBD is bound by the corepressors SMRT and NCoR, and has no access to the target  Sp1-binding GC boxes in the promoters or the enhancers.	bind
39303	10	9175	5	13	NULL	NULL	NULL	statement 2	GP		does not have access to					statement 6	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_30_28061_s_305	15878880	A and  B, Sp1ZFDBD is bound by the corepressors SMRT and NCoR, and has no access to the target  Sp1-binding GC boxes in the promoters or the enhancers.	bind
39304	11	9175	5	13	NULL	NULL	NULL	statement 5	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_30_28061_s_305	15878880	A and  B, Sp1ZFDBD is bound by the corepressors SMRT and NCoR, and has no access to the target  Sp1-binding GC boxes in the promoters or the enhancers.	bind
48040	5	9175	5	13	NULL	NULL	NULL	Sp-1	GP		bind									GC boxes in promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_30_28061_s_305	15878880	A and  B, Sp1ZFDBD is bound by the corepressors SMRT and NCoR, and has no access to the target  Sp1-binding GC boxes in the promoters or the enhancers.	bind
48041	6	9175	5	13	NULL	NULL	NULL	Sp-1	GP		bind									GC boxes in enhancer	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_30_28061_s_305	15878880	A and  B, Sp1ZFDBD is bound by the corepressors SMRT and NCoR, and has no access to the target  Sp1-binding GC boxes in the promoters or the enhancers.	bind
31812	1	9175	6	NULL	NULL	0	NULL	Sp1	NULL		bind	NULL		ZFDBD		SMRT	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_30_28061_s_305	15878880	A and  B, Sp1ZFDBD is bound by the corepressors SMRT and NCoR, and has no access to the target  Sp1-binding GC boxes in the promoters or the enhancers.	bind
31813	2	9175	6	NULL	NULL	0	NULL	Sp1	NULL		bind	NULL		ZFDBD		NcoR	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_30_28061_s_305	15878880	A and  B, Sp1ZFDBD is bound by the corepressors SMRT and NCoR, and has no access to the target  Sp1-binding GC boxes in the promoters or the enhancers.	bind
31814	3	9175	6	NULL	NULL	0	NULL	SMRT	NULL		is a type of	NULL				corepressor	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_30_28061_s_305	15878880	A and  B, Sp1ZFDBD is bound by the corepressors SMRT and NCoR, and has no access to the target  Sp1-binding GC boxes in the promoters or the enhancers.	bind
31815	4	9175	6	NULL	NULL	0	NULL	NcoR	NULL		is a type of	NULL				corepressor	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_30_28061_s_305	15878880	A and  B, Sp1ZFDBD is bound by the corepressors SMRT and NCoR, and has no access to the target  Sp1-binding GC boxes in the promoters or the enhancers.	bind
31816	6	9175	6	10	NULL	0	NULL	Sp1	NULL		bind	NULL					NULL			 GC boxes in the enhancer	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_30_28061_s_305	15878880	A and  B, Sp1ZFDBD is bound by the corepressors SMRT and NCoR, and has no access to the target  Sp1-binding GC boxes in the promoters or the enhancers.	bind
31817	7	9175	6	10	NULL	0	NULL	statement 1	NULL		has no access to	NULL				statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_30_28061_s_305	15878880	A and  B, Sp1ZFDBD is bound by the corepressors SMRT and NCoR, and has no access to the target  Sp1-binding GC boxes in the promoters or the enhancers.	bind
31818	8	9175	6	10	NULL	0	NULL	statement 1	NULL		has no access to	NULL				statement 6	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_30_28061_s_305	15878880	A and  B, Sp1ZFDBD is bound by the corepressors SMRT and NCoR, and has no access to the target  Sp1-binding GC boxes in the promoters or the enhancers.	bind
31819	9	9175	6	10	NULL	0	NULL	statement 2	NULL		has no access to	NULL				statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_30_28061_s_305	15878880	A and  B, Sp1ZFDBD is bound by the corepressors SMRT and NCoR, and has no access to the target  Sp1-binding GC boxes in the promoters or the enhancers.	bind
31820	10	9175	6	10	NULL	0	NULL	statement 2	NULL		has no access to	NULL				statement 6	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_30_28061_s_305	15878880	A and  B, Sp1ZFDBD is bound by the corepressors SMRT and NCoR, and has no access to the target  Sp1-binding GC boxes in the promoters or the enhancers.	bind
31821	11	9175	6	10	NULL	0	NULL	statement 5	NULL		is an alternative to	NULL				statement 6	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_30_28061_s_305	15878880	A and  B, Sp1ZFDBD is bound by the corepressors SMRT and NCoR, and has no access to the target  Sp1-binding GC boxes in the promoters or the enhancers.	bind
48042	5	9175	6	10	NULL	0	NULL	Sp1	NULL		bind	NULL					NULL			GC box in promoter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_30_28061_s_305	15878880	A and  B, Sp1ZFDBD is bound by the corepressors SMRT and NCoR, and has no access to the target  Sp1-binding GC boxes in the promoters or the enhancers.	bind
39305	1	9176	5	13	NULL	NULL	NULL	FGF	GP		forms binary complex with					FGFR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_31_21511_s_72	10419453	A and  B, specificity of the AT-binding fraction of heparin for formation of an FGF-binding binary complex with FGFR.	bind
39306	2	9176	5	13	NULL	NULL	NULL	heparin	Chemical		is required for		specifically	AT-binding fraction of		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_31_21511_s_72	10419453	A and  B, specificity of the AT-binding fraction of heparin for formation of an FGF-binding binary complex with FGFR.	bind
31822	1	9176	6	10	NULL	0	NULL	FGF 	NULL		forms binary complex with	NULL				FGFR	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_31_21511_s_72	10419453	A and  B, specificity of the AT-binding fraction of heparin for formation of an FGF-binding binary complex with FGFR.	bind
48043	2	9176	6	10	NULL	0	NULL	heparin	NULL		is required for	NULL	specifically	AT-binding fraction of 		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_31_21511_s_72	10419453	A and  B, specificity of the AT-binding fraction of heparin for formation of an FGF-binding binary complex with FGFR.	bind
39446	1	9179	5	13	NULL	NULL	NULL	p53	GP	wild type	bind					p21WAF1/CIP1	NucleicAcid			consensus DNA binding sites in promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_35_32990_s_243	11395510	A and  B, wild type p53 binds the consensus DNA binding sites in the p21WAF1/CIP1 and Bax promoters.	bind
39447	2	9179	5	13	NULL	NULL	NULL	p53	GP	wild type	bind					Bax	NucleicAcid			consensus DNA binding sites in promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_35_32990_s_243	11395510	A and  B, wild type p53 binds the consensus DNA binding sites in the p21WAF1/CIP1 and Bax promoters.	bind
31823	1	9179	6	NULL	NULL	0	NULL	p53	NULL	wild type	bind	NULL				p21WAF1/CIP1	NULL			DNA binding site of promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_35_32990_s_243	11395510	A and  B, wild type p53 binds the consensus DNA binding sites in the p21WAF1/CIP1 and Bax promoters.	bind
31824	2	9179	6	NULL	NULL	0	NULL	p53	NULL	wild type	bind	NULL				Bax	NULL			DNA binding site of promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_35_32990_s_243	11395510	A and  B, wild type p53 binds the consensus DNA binding sites in the p21WAF1/CIP1 and Bax promoters.	bind
39448	1	9180	5	13	NULL	NULL	NULL	spermine	Chemical		bind					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_47_30939_s_114	9812989	A and  C, binding constants of spermine for ATP without and with 1 mM Mg2+, respectively.	bind
31825	1	9180	6	NULL	NULL	0	NULL	spermine	NULL		bind	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_47_30939_s_114	9812989	A and  C, binding constants of spermine for ATP without and with 1 mM Mg2+, respectively.	bind
39449	1	9181	5	13	NULL	NULL	NULL	MM6.15 mAb	GP	Cy5 labeled	bind		specifically			Pgp molecules	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_315_4_942_s_85	14985103	A and B are internal controls  demonstrating that the Cy5 labeled MM6.15 mAb binds specifically to the Pgp molecules.	bind
31826	1	9181	6	NULL	NULL	0	NULL	MM6.15 mAb	NULL	Cy5 labeled	bind	NULL	specifically			Pgp molecules	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_315_4_942_s_85	14985103	A and B are internal controls  demonstrating that the Cy5 labeled MM6.15 mAb binds specifically to the Pgp molecules.	bind
39450	1	9182	5	13	NULL	NULL	NULL	RyhB	NucleicAcid		mediates					sodB mRNA	NucleicAcid	degradation of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_19_2374_s_69	12975324	A and B), indicating that RNase III is not required for RyhB-mediated  sodB mRNA degradation.	bind
39451	2	9182	5	13	NULL	NULL	NULL	RNase III	GP		is not required for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_19_2374_s_69	12975324	A and B), indicating that RNase III is not required for RyhB-mediated  sodB mRNA degradation.	bind
31827	1	9182	6	NULL	NULL	0	NULL	RyhB	NULL		mediates	NULL				sodB mRNA	NULL	degradation of			NULL		0	NULL	NULL	NULL	gw70_genesdev_17_19_2374_s_69	12975324	A and B), indicating that RNase III is not required for RyhB-mediated  sodB mRNA degradation.	bind
31828	2	9182	6	NULL	NULL	0	NULL	RNase III	NULL		is not required for	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_17_19_2374_s_69	12975324	A and B), indicating that RNase III is not required for RyhB-mediated  sodB mRNA degradation.	bind
39452	1	9184	5	13	NULL	NULL	NULL	TCDD-inducible protein	GP		bind					HES-1	GP			XRE element present in flanking region	NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_65_1_165_s_116	14722248	A and B, a TCDD-inducible protein binds the XRE element present in the HES-1 flanking  region.	bind
31829	1	9184	6	10	NULL	0	NULL	TCDD-inducible protein	NULL		bind	NULL				HES-1	NULL			XRE element in the  flanking region	NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_65_1_165_s_116	14722248	A and B, a TCDD-inducible protein binds the XRE element present in the HES-1 flanking  region.	bind
39453	1	9185	5	13	NULL	NULL	NULL	EB	Chemical		bind					splenocytes	Cell	mice			NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_66_6_1712_s_118	15383622	A and B, ligand-binding isotherms and Scatchard plots (insets) of [3]EB and 125I-alpha-BGT binding to mice splenocytes ( n = 3).	bind
39454	2	9185	5	13	NULL	NULL	NULL	alpha-BGT	Chemical	125I	bind					splenocytes	Cell	mice			NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_66_6_1712_s_118	15383622	A and B, ligand-binding isotherms and Scatchard plots (insets) of [3]EB and 125I-alpha-BGT binding to mice splenocytes ( n = 3).	bind
31830	1	9185	6	NULL	NULL	0	NULL	EB	NULL		bind	NULL				splenocytes	NULL	mice			NULL		0	NULL	NULL	NULL	gw70_molpharmacol_66_6_1712_s_118	15383622	A and B, ligand-binding isotherms and Scatchard plots (insets) of [3]EB and 125I-alpha-BGT binding to mice splenocytes ( n = 3).	bind
31831	2	9185	6	10	NULL	0	NULL	alpha-BGT		125I	bind					splenocytes		mice			NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_66_6_1712_s_118	15383622	A and B, ligand-binding isotherms and Scatchard plots (insets) of [3]EB and 125I-alpha-BGT binding to mice splenocytes ( n = 3).	bind
39455	1	9186	5	13	NULL	NULL	NULL	TRAX	GP		bind					A2A-R	GP	striatal			NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_70_2_454_s_181	16617164	A and B, TRAX bound the striatal  A2A-R in GST pull-down assays.	bind
31832	1	9186	6	NULL	NULL	0	NULL	TRAX	NULL		bind	NULL				A2A-R	NULL	striatal			NULL		0	NULL	NULL	NULL	gw70_molpharmacol_70_2_454_s_181	16617164	A and B, TRAX bound the striatal  A2A-R in GST pull-down assays.	bind
39456	1	9187	5	13	NULL	NULL	NULL	NGF	GP		is relocated inside					cytoplasm	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_neurobioldis_15_1_106_s_167	14751775	A and C. NGF was relocated inside the cytoplasm, presumably bound to TrkA receptors.	bind
39457	2	9187	5	13	NULL	NULL	NULL	statement 1	GP		bind		presumably			TrkA receptors	GP				NULL		NULL	NULL	NULL	NULL	gw70_neurobioldis_15_1_106_s_167	14751775	A and C. NGF was relocated inside the cytoplasm, presumably bound to TrkA receptors.	bind
31833	1	9187	6	NULL	NULL	0	NULL	NGF	NULL		bind	NULL	presumably			TrkA receptor	NULL				NULL		0	NULL	NULL	NULL	gw70_neurobioldis_15_1_106_s_167	14751775	A and C. NGF was relocated inside the cytoplasm, presumably bound to TrkA receptors.	bind
31834	2	9187	6	NULL	NULL	0	NULL	statement 1	NULL		relocates inside	NULL				cytoplasm	NULL				NULL		0	NULL	NULL	NULL	gw70_neurobioldis_15_1_106_s_167	14751775	A and C. NGF was relocated inside the cytoplasm, presumably bound to TrkA receptors.	bind
39458	1	9188	5	13	NULL	NULL	NULL	ATP	Chemical		bind					A2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_46_29255_s_50	9361005	A and CPS.B. Chemical modification of CAD ( 41) and mammalian CPSase I ( 40,  42-45) as well as site-directed mutagenesis of  E. coli CPSase ( 23,  46,  47) showed that ATP binds to A2 and B2.	bind
39459	2	9188	5	13	NULL	NULL	NULL	ATP	Chemical		bind					B2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_46_29255_s_50	9361005	A and CPS.B. Chemical modification of CAD ( 41) and mammalian CPSase I ( 40,  42-45) as well as site-directed mutagenesis of  E. coli CPSase ( 23,  46,  47) showed that ATP binds to A2 and B2.	bind
31835	1	9188	6	NULL	NULL	0	NULL	ATP	NULL		bind	NULL				A2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_46_29255_s_50	9361005	A and CPS.B. Chemical modification of CAD ( 41) and mammalian CPSase I ( 40,  42-45) as well as site-directed mutagenesis of  E. coli CPSase ( 23,  46,  47) showed that ATP binds to A2 and B2.	bind
31836	2	9188	6	NULL	NULL	0	NULL	ATP	NULL		bind	NULL				B2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_46_29255_s_50	9361005	A and CPS.B. Chemical modification of CAD ( 41) and mammalian CPSase I ( 40,  42-45) as well as site-directed mutagenesis of  E. coli CPSase ( 23,  46,  47) showed that ATP binds to A2 and B2.	bind
39466	1	9189	5	13	NULL	NULL	NULL	ATP	Chemical		bind					F-6-P	Chemical				NULL	E. coli ATP-PFK enzyme	NULL	NULL	NULL	NULL	gw60_jbacteriol_183_24_7231_s_217	11717283	A and F indicate residues (solid boxes) involved in binding of ATP and F-6-P, respectively, in the  E. coli ATP-PFK enzyme ( 34).	bind
31837	1	9189	6	NULL	NULL	0	NULL	ATP	NULL		bind	NULL				F-6-P	NULL				NULL	E. coli ATP-PFK enzyme	0	NULL	NULL	NULL	gw60_jbacteriol_183_24_7231_s_217	11717283	A and F indicate residues (solid boxes) involved in binding of ATP and F-6-P, respectively, in the  E. coli ATP-PFK enzyme ( 34).	bind
39468	1	9190	5	13	NULL	NULL	NULL	B cell	Cell		bind					autoantigen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_5_2_103_s_67	7743168	A B cell that has bound an autoantigen is very unlikely to find a specific helper T cell, for autoreactive T cells are normally eliminated by a rigorous selection process  [10]  .	bind
39469	2	9190	5	13	NULL	NULL	NULL	statement 1	Chemical		does not find					helper T cell	Cell	specific			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_5_2_103_s_67	7743168	A B cell that has bound an autoantigen is very unlikely to find a specific helper T cell, for autoreactive T cells are normally eliminated by a rigorous selection process  [10]  .	bind
39476	3	9190	5	13	NULL	NULL	NULL	T cells	Cell	autoreactive	eliminated by		normally			selection process	Process	rigorous			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_5_2_103_s_67	7743168	A B cell that has bound an autoantigen is very unlikely to find a specific helper T cell, for autoreactive T cells are normally eliminated by a rigorous selection process  [10]  .	bind
31838	1	9190	6	NULL	NULL	0	NULL	B cell 	NULL		bind	NULL				autoantigen	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_5_2_103_s_67	7743168	A B cell that has bound an autoantigen is very unlikely to find a specific helper T cell, for autoreactive T cells are normally eliminated by a rigorous selection process  [10]  .	bind
31839	2	9190	6	10	NULL	0	NULL	T cells		autoreactive	are eliminated		normally			 selection process		rigorous			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_5_2_103_s_67	7743168	A B cell that has bound an autoantigen is very unlikely to find a specific helper T cell, for autoreactive T cells are normally eliminated by a rigorous selection process  [10]  .	bind
31840	3	9190	6	NULL	NULL	0	NULL	statement 1	NULL		does not find	NULL				helper T cell	NULL	specific			NULL		0	NULL	NULL	NULL	gw60_currbiol_5_2_103_s_67	7743168	A B cell that has bound an autoantigen is very unlikely to find a specific helper T cell, for autoreactive T cells are normally eliminated by a rigorous selection process  [10]  .	bind
39478	1	9191	5	13	NULL	NULL	NULL	nuclear factor	GP	B-cell-specific	bind					RAG-2	NucleicAcid			core promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_2601_s_243	10082526	A B-cell-specific nuclear factor binds to the core  RAG-2 promoter.	bind
31841	1	9191	6	10	NULL	0	NULL	nuclear factor	NULL	B-cell specific	bind	NULL				RAG-2 	NULL			core promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_2601_s_243	10082526	A B-cell-specific nuclear factor binds to the core  RAG-2 promoter.	bind
39539	1	9192	5	13	NULL	NULL	NULL	mAb 6B2	GP		bind					CD45	GP	glycosylation variant of			NULL		NULL	NULL	NULL	NULL	gw70_microbesinfect_5_3_205_s_179	12681409	A B220- memory fraction (mAb 6B2 binding of a glycosylation variant of CD45) (B220- CD19- CD11b+ CD43+) divides again based on IgG or IgE expression [  47 and   48].	bind
31842	1	9192	6	NULL	NULL	0	NULL	CD45	NULL	glycosylation variant of	bind	NULL				6B2 mAb	NULL				NULL		0	NULL	NULL	NULL	gw70_microbesinfect_5_3_205_s_179	12681409	A B220- memory fraction (mAb 6B2 binding of a glycosylation variant of CD45) (B220- CD19- CD11b+ CD43+) divides again based on IgG or IgE expression [  47 and   48].	bind
39540	2	9193	5	13	NULL	NULL	NULL	B7x-Ig	GP		bind					statement 1	Cell				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_18_10388_s_25	12920180	A B7x-Ig fusion protein binds to  Th1 cells derived from WT mice, but not mice with induced null mutation for  the newly identified CD28 homolog BTLA (B and T lymphocyte attenuator)  ( ).	bind
39541	1	9193	5	13	NULL	NULL	NULL	Th1 cells	Cell		is derived from					mice	Organism	WT			NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_18_10388_s_25	12920180	A B7x-Ig fusion protein binds to  Th1 cells derived from WT mice, but not mice with induced null mutation for  the newly identified CD28 homolog BTLA (B and T lymphocyte attenuator)  ( ).	bind
48044	3	9193	5	13	NULL	NULL	NULL	Th1 cells	Cell		derived from					mice	Organism	null mutant			NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_18_10388_s_25	12920180	A B7x-Ig fusion protein binds to  Th1 cells derived from WT mice, but not mice with induced null mutation for  the newly identified CD28 homolog BTLA (B and T lymphocyte attenuator)  ( ).	bind
48045	4	9193	5	13	NULL	NULL	NULL	B7x-Ig 	GP		does not bind					statement 3	Cell				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_18_10388_s_25	12920180	A B7x-Ig fusion protein binds to  Th1 cells derived from WT mice, but not mice with induced null mutation for  the newly identified CD28 homolog BTLA (B and T lymphocyte attenuator)  ( ).	bind
48046	5	9193	5	13	NULL	NULL	NULL	 B7x-Ig	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_18_10388_s_25	12920180	A B7x-Ig fusion protein binds to  Th1 cells derived from WT mice, but not mice with induced null mutation for  the newly identified CD28 homolog BTLA (B and T lymphocyte attenuator)  ( ).	bind
48047	6	9193	5	13	NULL	NULL	NULL	BTLA	GP		is					B and T lymphocyte attenuator	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_18_10388_s_25	12920180	A B7x-Ig fusion protein binds to  Th1 cells derived from WT mice, but not mice with induced null mutation for  the newly identified CD28 homolog BTLA (B and T lymphocyte attenuator)  ( ).	bind
31843	1	9193	6	NULL	NULL	0	NULL	Th1 cells	NULL		are derived from	NULL				mice	NULL	WT			NULL		0	NULL	NULL	NULL	gw70_pnas_100_18_10388_s_25	12920180	A B7x-Ig fusion protein binds to  Th1 cells derived from WT mice, but not mice with induced null mutation for  the newly identified CD28 homolog BTLA (B and T lymphocyte attenuator)  ( ).	bind
31844	2	9193	6	10	NULL	0	NULL	B7x-Ig	NULL		bind	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_18_10388_s_25	12920180	A B7x-Ig fusion protein binds to  Th1 cells derived from WT mice, but not mice with induced null mutation for  the newly identified CD28 homolog BTLA (B and T lymphocyte attenuator)  ( ).	bind
31845	3	9193	6	NULL	NULL	0	NULL	Th1	NULL		derived from	NULL				mice	NULL	null mutant			NULL		0	NULL	NULL	NULL	gw70_pnas_100_18_10388_s_25	12920180	A B7x-Ig fusion protein binds to  Th1 cells derived from WT mice, but not mice with induced null mutation for  the newly identified CD28 homolog BTLA (B and T lymphocyte attenuator)  ( ).	bind
31846	4	9193	6	10	NULL	0	NULL	B7x-Ig 	NULL		does not bind	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_18_10388_s_25	12920180	A B7x-Ig fusion protein binds to  Th1 cells derived from WT mice, but not mice with induced null mutation for  the newly identified CD28 homolog BTLA (B and T lymphocyte attenuator)  ( ).	bind
31847	5	9193	6	NULL	NULL	0	NULL	BTLA	NULL		is	NULL				B and T lymphocyte attenuator	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_100_18_10388_s_25	12920180	A B7x-Ig fusion protein binds to  Th1 cells derived from WT mice, but not mice with induced null mutation for  the newly identified CD28 homolog BTLA (B and T lymphocyte attenuator)  ( ).	bind
48048	6	9193	6	10	NULL	0	NULL	B7x-Ig	NULL		is a type of	NULL				fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_100_18_10388_s_25	12920180	A B7x-Ig fusion protein binds to  Th1 cells derived from WT mice, but not mice with induced null mutation for  the newly identified CD28 homolog BTLA (B and T lymphocyte attenuator)  ( ).	bind
39542	1	9194	5	13	NULL	NULL	NULL	IgA-Fc-binding protein	GP	bacterial	is unrelated to					Sir22	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14521_s_148	10329638	A bacterial IgA-Fc-binding protein unrelated to Sir22 has been described in group B streptococcus ( 5,  23,  24), and a fusion protein including a 73-residue sequence from this protein was found to bind IgA ( 25).	bind
39543	2	9194	5	13	NULL	NULL	NULL	statement 1	GP		is described in					group B streptococcus	Organism				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14521_s_148	10329638	A bacterial IgA-Fc-binding protein unrelated to Sir22 has been described in group B streptococcus ( 5,  23,  24), and a fusion protein including a 73-residue sequence from this protein was found to bind IgA ( 25).	bind
39544	3	9194	5	13	NULL	NULL	NULL	fusion protein	GP		include					IgA-Fc-binding protein	GP	73-residue sequence from			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14521_s_148	10329638	A bacterial IgA-Fc-binding protein unrelated to Sir22 has been described in group B streptococcus ( 5,  23,  24), and a fusion protein including a 73-residue sequence from this protein was found to bind IgA ( 25).	bind
39545	4	9194	5	13	NULL	NULL	NULL	statement 3	GP		bind					IgA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14521_s_148	10329638	A bacterial IgA-Fc-binding protein unrelated to Sir22 has been described in group B streptococcus ( 5,  23,  24), and a fusion protein including a 73-residue sequence from this protein was found to bind IgA ( 25).	bind
32030	1	9194	6	NULL	NULL	0	NULL	IgA-Fc-binding protein	NULL	bacterial	bind	NULL		73 residue sequence		IgA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_21_14521_s_148	10329638	A bacterial IgA-Fc-binding protein unrelated to Sir22 has been described in group B streptococcus ( 5,  23,  24), and a fusion protein including a 73-residue sequence from this protein was found to bind IgA ( 25).	bind
32824	2	9194	6	NULL	NULL	0	NULL	IgA-Fc-binding protein	NULL		is unrelated to	NULL				Sir22	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_21_14521_s_148	10329638	A bacterial IgA-Fc-binding protein unrelated to Sir22 has been described in group B streptococcus ( 5,  23,  24), and a fusion protein including a 73-residue sequence from this protein was found to bind IgA ( 25).	bind
57851	3	9194	6	10	NULL	0	NULL	statement 2			is described in					group B streptococcus					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14521_s_148	10329638	A bacterial IgA-Fc-binding protein unrelated to Sir22 has been described in group B streptococcus ( 5,  23,  24), and a fusion protein including a 73-residue sequence from this protein was found to bind IgA ( 25).	bind
39546	1	9198	5	13	NULL	NULL	NULL	POP-1 fragment	GP	bacterially expressed	bind		specifically	HMG domain				optimal		 Tcf target site	NULL		NULL	NULL	NULL	NULL	gw60_nature_406_6795_527_s_32	10952315	A bacterially expressed POP-1 fragment containing the HMG domain specifically binds the optimal Tcf target site, but not a sequence that lacks the core Tcf target motif ( Fig. 1a).	bind
39547	3	9198	5	13	NULL	NULL	NULL	POP-1 fragment	GP	bacterially expressed	does not bind			HMG domain		statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_nature_406_6795_527_s_32	10952315	A bacterially expressed POP-1 fragment containing the HMG domain specifically binds the optimal Tcf target site, but not a sequence that lacks the core Tcf target motif ( Fig. 1a).	bind
48049	2	9198	5	13	NULL	NULL	NULL	sequence	GP		lacks								 core Tcf target motif		NULL		NULL	NULL	NULL	NULL	gw60_nature_406_6795_527_s_32	10952315	A bacterially expressed POP-1 fragment containing the HMG domain specifically binds the optimal Tcf target site, but not a sequence that lacks the core Tcf target motif ( Fig. 1a).	bind
32031	1	9198	6	NULL	NULL	0	NULL	POP-1 fragment	NULL	bacterially expressed	bind	NULL	specifically	HMG domain			NULL	optimal		Tcf target site	NULL		0	NULL	NULL	NULL	gw60_nature_406_6795_527_s_32	10952315	A bacterially expressed POP-1 fragment containing the HMG domain specifically binds the optimal Tcf target site, but not a sequence that lacks the core Tcf target motif ( Fig. 1a).	bind
48050	2	9198	6	10	NULL	0	NULL	sequence	NULL		lacks	NULL					NULL		 core Tcf target motif		NULL		0	NULL	NULL	NULL	gw60_nature_406_6795_527_s_32	10952315	A bacterially expressed POP-1 fragment containing the HMG domain specifically binds the optimal Tcf target site, but not a sequence that lacks the core Tcf target motif ( Fig. 1a).	bind
48051	3	9198	6	10	NULL	0	NULL	POP-1 fragment	NULL	bacterially expressed	does not bind	NULL		HMG domain		statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_nature_406_6795_527_s_32	10952315	A bacterially expressed POP-1 fragment containing the HMG domain specifically binds the optimal Tcf target site, but not a sequence that lacks the core Tcf target motif ( Fig. 1a).	bind
39548	1	9201	5	13	NULL	NULL	NULL	Bak BH3 peptide	GP		antagonize					Bcl-xL	GP	protective effects of 			NULL	alpha-Fas-treated HeLa cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_19_13298_s_17	10224090	A Bak BH3 peptide was found to antagonize the protective effects of microinjected Bcl-xL in alpha-Fas-treated HeLa cells, whereas a mutant Bak BH3 peptide that no longerR binds Bcl-xL was inactive.	bind
39549	2	9201	5	13	NULL	NULL	NULL	Bak BH3 peptide	GP	mutant	does not bind					Bcl-xL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_19_13298_s_17	10224090	A Bak BH3 peptide was found to antagonize the protective effects of microinjected Bcl-xL in alpha-Fas-treated HeLa cells, whereas a mutant Bak BH3 peptide that no longerR binds Bcl-xL was inactive.	bind
49531	3	9201	5	13	NULL	NULL	NULL	Bak BH3 peptide	GP		bind					Bcl-xL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_19_13298_s_17	10224090	A Bak BH3 peptide was found to antagonize the protective effects of microinjected Bcl-xL in alpha-Fas-treated HeLa cells, whereas a mutant Bak BH3 peptide that no longerR binds Bcl-xL was inactive.	bind
32032	1	9201	6	NULL	NULL	0	NULL	Bak BH3 peptide	NULL		bind	NULL				Bcl-xL	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_19_13298_s_17	10224090	A Bak BH3 peptide was found to antagonize the protective effects of microinjected Bcl-xL in alpha-Fas-treated HeLa cells, whereas a mutant Bak BH3 peptide that no longerR binds Bcl-xL was inactive.	bind
32034	2	9201	6	10	NULL	0	NULL	Bak BH3 peptide	NULL		antagonizes	NULL				Bcl-xL	NULL	protective effects of 			NULL	alpha-Fas-treated HeLa cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_19_13298_s_17	10224090	A Bak BH3 peptide was found to antagonize the protective effects of microinjected Bcl-xL in alpha-Fas-treated HeLa cells, whereas a mutant Bak BH3 peptide that no longerR binds Bcl-xL was inactive.	bind
32035	3	9201	6	10	NULL	0	NULL	Bak BH3 peptide	NULL	mutant	does not bind	NULL				Bcl-xL	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_19_13298_s_17	10224090	A Bak BH3 peptide was found to antagonize the protective effects of microinjected Bcl-xL in alpha-Fas-treated HeLa cells, whereas a mutant Bak BH3 peptide that no longerR binds Bcl-xL was inactive.	bind
39551	1	9202	5	13	NULL	NULL	NULL	180 kDa protein	GP		bind		specifically			NR2A	GP				NULL	WT tissue	NULL	NULL	NULL	NULL	gw70_jneurosci_24_49_11098_s_85	15590926	A band corresponding  to 180 kDa was detected in the lane containing WT but not NR2AKO tissue (arrowhead)  demonstrating specific binding to NR2A and no cross-reactivity with NR2B.	bind
39552	2	9202	5	13	NULL	NULL	NULL	statement 1	GP		does not cross react with					NR2B	GP				NULL		NULL	NULL	NULL	NULL	gw70_jneurosci_24_49_11098_s_85	15590926	A band corresponding  to 180 kDa was detected in the lane containing WT but not NR2AKO tissue (arrowhead)  demonstrating specific binding to NR2A and no cross-reactivity with NR2B.	bind
32037	1	9202	6	NULL	NULL	0	NULL	protein 180kDa	NULL		bind	NULL	specifically			NR2A	NULL				NULL		0	NULL	NULL	NULL	gw70_jneurosci_24_49_11098_s_85	15590926	A band corresponding  to 180 kDa was detected in the lane containing WT but not NR2AKO tissue (arrowhead)  demonstrating specific binding to NR2A and no cross-reactivity with NR2B.	bind
32038	2	9202	6	10	NULL	0	NULL	 180kDa protein	NULL		does not cross react with	NULL				NR2B	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jneurosci_24_49_11098_s_85	15590926	A band corresponding  to 180 kDa was detected in the lane containing WT but not NR2AKO tissue (arrowhead)  demonstrating specific binding to NR2A and no cross-reactivity with NR2B.	bind
39553	1	9203	5	13	NULL	NULL	NULL	20 kDa protein	GP		bind					calmodulin	GP	high concentrations of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_27_24500_s_168	12716903	A band of  unknown nature migrating at the front of the gel (<20 kDa) bound calmodulin  when the latter was present in high concentrations, but the binding persisted,  albeit weakly, in the presence of EGTA.	bind
39554	2	9203	5	13	NULL	NULL	NULL	statement 1	Process		persists		weakly			EGTA	Chemical	in presence of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_27_24500_s_168	12716903	A band of  unknown nature migrating at the front of the gel (<20 kDa) bound calmodulin  when the latter was present in high concentrations, but the binding persisted,  albeit weakly, in the presence of EGTA.	bind
39555	1	9204	5	13	NULL	NULL	NULL	30 kDa band	GP		corresponds to							size of	B subunit		NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_12_7623_s_114	10075648	A band of about 30 kDa, corresponding to the size of the B subunit  in vivo (Fig.  3,  lane NE), binds p300, which confirms the data obtained  in vitro (compare Figs.  2 and  3).	bind
39556	2	9204	5	13	NULL	NULL	NULL	statement 1	GP		bind					p300	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_12_7623_s_114	10075648	A band of about 30 kDa, corresponding to the size of the B subunit  in vivo (Fig.  3,  lane NE), binds p300, which confirms the data obtained  in vitro (compare Figs.  2 and  3).	bind
32039	1	9204	6	10	NULL	0	NULL	30kDa	NULL		bind	NULL				p300	NULL				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_12_7623_s_114	10075648	A band of about 30 kDa, corresponding to the size of the B subunit  in vivo (Fig.  3,  lane NE), binds p300, which confirms the data obtained  in vitro (compare Figs.  2 and  3).	bind
48052	2	9204	6	10	NULL	0	NULL	30 kDa	NULL		corresponds to	NULL					NULL	size of	B subunit		NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_12_7623_s_114	10075648	A band of about 30 kDa, corresponding to the size of the B subunit  in vivo (Fig.  3,  lane NE), binds p300, which confirms the data obtained  in vitro (compare Figs.  2 and  3).	bind
39630	1	9205	5	13	NULL	NULL	NULL	 Tenascin-C	GP		bind			 C terminus		Heparin	Chemical		C terminus of fibrinogen-like domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_7_3378_s_188	7531705	A Basic Peptide from the Extreme C Terminus of Tenascin-C  Binds to Heparin At the C terminus of the fibrinogen-like  domain, and hence at extreme end of the coding sequence of tenascin-C,  a conspicuous stretch of basic amino acids is found which is conserved  among species (but which is not found in fibrinogen itself).	bind
39631	2	9205	5	13	NULL	NULL	NULL	tenascin-C	GP		contains			extreme end of coding sequence of		basic amino acids	AminoAcid	conspicuous stretch of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_7_3378_s_188	7531705	A Basic Peptide from the Extreme C Terminus of Tenascin-C  Binds to Heparin At the C terminus of the fibrinogen-like  domain, and hence at extreme end of the coding sequence of tenascin-C,  a conspicuous stretch of basic amino acids is found which is conserved  among species (but which is not found in fibrinogen itself).	bind
39633	3	9205	5	13	NULL	NULL	NULL	statement 2	AminoAcid		is conserved among					species	Organism				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_7_3378_s_188	7531705	A Basic Peptide from the Extreme C Terminus of Tenascin-C  Binds to Heparin At the C terminus of the fibrinogen-like  domain, and hence at extreme end of the coding sequence of tenascin-C,  a conspicuous stretch of basic amino acids is found which is conserved  among species (but which is not found in fibrinogen itself).	bind
39634	4	9205	5	13	NULL	NULL	NULL	statement 2	AminoAcid		is not found in					fibrinogen	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_7_3378_s_188	7531705	A Basic Peptide from the Extreme C Terminus of Tenascin-C  Binds to Heparin At the C terminus of the fibrinogen-like  domain, and hence at extreme end of the coding sequence of tenascin-C,  a conspicuous stretch of basic amino acids is found which is conserved  among species (but which is not found in fibrinogen itself).	bind
32559	1	9205	6	10	NULL	0	NULL	Tenascin-C	NULL		bind	NULL		C-terminus		heparin	NULL		C terminus of the fibrinogen-like domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_7_3378_s_188	7531705	A Basic Peptide from the Extreme C Terminus of Tenascin-C  Binds to Heparin At the C terminus of the fibrinogen-like  domain, and hence at extreme end of the coding sequence of tenascin-C,  a conspicuous stretch of basic amino acids is found which is conserved  among species (but which is not found in fibrinogen itself).	bind
57852	2	9205	6	10	NULL	0	NULL	tenascin-C			contains			extreme end of the coding sequence of 		basic amino acids		conspicuous stretch of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_7_3378_s_188	7531705	A Basic Peptide from the Extreme C Terminus of Tenascin-C  Binds to Heparin At the C terminus of the fibrinogen-like  domain, and hence at extreme end of the coding sequence of tenascin-C,  a conspicuous stretch of basic amino acids is found which is conserved  among species (but which is not found in fibrinogen itself).	bind
57853	3	9205	6	10	NULL	0	NULL	statement 2			is conserved among					species					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_7_3378_s_188	7531705	A Basic Peptide from the Extreme C Terminus of Tenascin-C  Binds to Heparin At the C terminus of the fibrinogen-like  domain, and hence at extreme end of the coding sequence of tenascin-C,  a conspicuous stretch of basic amino acids is found which is conserved  among species (but which is not found in fibrinogen itself).	bind
57854	4	9205	6	10	NULL	0	NULL	statement 2			is not found in					fibrinogen					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_7_3378_s_188	7531705	A Basic Peptide from the Extreme C Terminus of Tenascin-C  Binds to Heparin At the C terminus of the fibrinogen-like  domain, and hence at extreme end of the coding sequence of tenascin-C,  a conspicuous stretch of basic amino acids is found which is conserved  among species (but which is not found in fibrinogen itself).	bind
39635	1	9206	5	13	NULL	NULL	NULL				bind		differentially	SHP motif		LRH-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_27_9505_s_208	15976031	A basis for the differential binding of the SHP motif to LRH-1 and SF-1 becomes evident by comparing the surface topology of their coactivator-binding sites ( Fig. 5).	bind
39636	2	9206	5	13	NULL	NULL	NULL				bind		differentially	SHP motif		SF-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_27_9505_s_208	15976031	A basis for the differential binding of the SHP motif to LRH-1 and SF-1 becomes evident by comparing the surface topology of their coactivator-binding sites ( Fig. 5).	bind
32040	1	9206	6	NULL	NULL	0	NULL		NULL		bind	NULL	differentially	SHP motif		LRH-1	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_27_9505_s_208	15976031	A basis for the differential binding of the SHP motif to LRH-1 and SF-1 becomes evident by comparing the surface topology of their coactivator-binding sites ( Fig. 5).	bind
32041	2	9206	6	NULL	NULL	0	NULL		NULL		bind	NULL	differentially	SHP motif		SF-1	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_27_9505_s_208	15976031	A basis for the differential binding of the SHP motif to LRH-1 and SF-1 becomes evident by comparing the surface topology of their coactivator-binding sites ( Fig. 5).	bind
39637	1	9207	5	13	NULL	NULL	NULL	BCR pY177 peptide	GP		is					Lys-Pro-Phe- Tyr(P)-Val-Asn-Val-Glu-Phe	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_2_894_s_166	8995379	A BCR pY177 peptide (Lys-Pro-Phe- Tyr(P)-Val-Asn-Val-Glu-Phe) binds Grb2 and Grap SH2 domains with equivalent high affinity (ID50 = 2.1  plus-or-minus  0.4 muM and 0.8  plus-or-minus  0.3 muM, respectively).	bind
39638	2	9207	5	13	NULL	NULL	NULL	BCR pY177 peptide	GP		bind		high affinity			Grb2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_2_894_s_166	8995379	A BCR pY177 peptide (Lys-Pro-Phe- Tyr(P)-Val-Asn-Val-Glu-Phe) binds Grb2 and Grap SH2 domains with equivalent high affinity (ID50 = 2.1  plus-or-minus  0.4 muM and 0.8  plus-or-minus  0.3 muM, respectively).	bind
39639	3	9207	5	13	NULL	NULL	NULL	BCR pY177 peptide	GP		bind		high affinity			Grap	GP		SH2 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_2_894_s_166	8995379	A BCR pY177 peptide (Lys-Pro-Phe- Tyr(P)-Val-Asn-Val-Glu-Phe) binds Grb2 and Grap SH2 domains with equivalent high affinity (ID50 = 2.1  plus-or-minus  0.4 muM and 0.8  plus-or-minus  0.3 muM, respectively).	bind
39640	4	9207	5	13	NULL	NULL	NULL	statement 2	Process	affinity of	is equal to					statement 3	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_2_894_s_166	8995379	A BCR pY177 peptide (Lys-Pro-Phe- Tyr(P)-Val-Asn-Val-Glu-Phe) binds Grb2 and Grap SH2 domains with equivalent high affinity (ID50 = 2.1  plus-or-minus  0.4 muM and 0.8  plus-or-minus  0.3 muM, respectively).	bind
32042	1	9207	6	10	NULL	0	NULL	BCR pY177 peptide			bind		high affinity			Grb2					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_2_894_s_166	8995379	A BCR pY177 peptide (Lys-Pro-Phe- Tyr(P)-Val-Asn-Val-Glu-Phe) binds Grb2 and Grap SH2 domains with equivalent high affinity (ID50 = 2.1  plus-or-minus  0.4 muM and 0.8  plus-or-minus  0.3 muM, respectively).	bind
32043	2	9207	6	10	NULL	0	NULL	BCR pY177 peptide			bind		high affinity			Grap			SH2 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_2_894_s_166	8995379	A BCR pY177 peptide (Lys-Pro-Phe- Tyr(P)-Val-Asn-Val-Glu-Phe) binds Grb2 and Grap SH2 domains with equivalent high affinity (ID50 = 2.1  plus-or-minus  0.4 muM and 0.8  plus-or-minus  0.3 muM, respectively).	bind
32044	3	9207	6	NULL	NULL	0	NULL	statement 1	NULL	affinity of	is equal to	NULL				statement 2	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_2_894_s_166	8995379	A BCR pY177 peptide (Lys-Pro-Phe- Tyr(P)-Val-Asn-Val-Glu-Phe) binds Grb2 and Grap SH2 domains with equivalent high affinity (ID50 = 2.1  plus-or-minus  0.4 muM and 0.8  plus-or-minus  0.3 muM, respectively).	bind
32045	4	9207	6	NULL	NULL	0	NULL	BCR pY177 peptide	NULL		is	NULL				Lys-Pro-Phe- Tyr(P)-Val-Asn-Val-Glu-Phe	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_2_894_s_166	8995379	A BCR pY177 peptide (Lys-Pro-Phe- Tyr(P)-Val-Asn-Val-Glu-Phe) binds Grb2 and Grap SH2 domains with equivalent high affinity (ID50 = 2.1  plus-or-minus  0.4 muM and 0.8  plus-or-minus  0.3 muM, respectively).	bind
39641	1	9208	5	13	NULL	NULL	NULL	Bem1p	GP		bind		directly			Cla4p	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7176_s_310	11113154	A Bem1p-dependent Complex Containing Cdc24p, Cdc42p, and Cla4p--  We report that Bem1p binds directly to Cla4p and to GTP-Cdc42p as well as to Cdc24p and can mediate the assembly of complexes containing each of these proteins  in vitro.	bind
39642	2	9208	5	13	NULL	NULL	NULL	Bem1p	GP		bind		directly			GTP-Cdc42p	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7176_s_310	11113154	A Bem1p-dependent Complex Containing Cdc24p, Cdc42p, and Cla4p--  We report that Bem1p binds directly to Cla4p and to GTP-Cdc42p as well as to Cdc24p and can mediate the assembly of complexes containing each of these proteins  in vitro.	bind
39643	3	9208	5	13	NULL	NULL	NULL	Bem1p	GP		bind		directly			Cdc24p	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7176_s_310	11113154	A Bem1p-dependent Complex Containing Cdc24p, Cdc42p, and Cla4p--  We report that Bem1p binds directly to Cla4p and to GTP-Cdc42p as well as to Cdc24p and can mediate the assembly of complexes containing each of these proteins  in vitro.	bind
39644	4	9208	5	13	NULL	NULL	NULL	Bem1p	GP		mediate					Cdc24p	GP	assembly of complexes containing			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7176_s_310	11113154	A Bem1p-dependent Complex Containing Cdc24p, Cdc42p, and Cla4p--  We report that Bem1p binds directly to Cla4p and to GTP-Cdc42p as well as to Cdc24p and can mediate the assembly of complexes containing each of these proteins  in vitro.	bind
39645	5	9208	5	13	NULL	NULL	NULL	Bem1p	GP		mediate					GTP-Cdc42p	GP	assembly of complexes containing			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7176_s_310	11113154	A Bem1p-dependent Complex Containing Cdc24p, Cdc42p, and Cla4p--  We report that Bem1p binds directly to Cla4p and to GTP-Cdc42p as well as to Cdc24p and can mediate the assembly of complexes containing each of these proteins  in vitro.	bind
39646	6	9208	5	13	NULL	NULL	NULL	Bem1p	GP		mediate					Cla4p	GP	assembly of complexes containing			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7176_s_310	11113154	A Bem1p-dependent Complex Containing Cdc24p, Cdc42p, and Cla4p--  We report that Bem1p binds directly to Cla4p and to GTP-Cdc42p as well as to Cdc24p and can mediate the assembly of complexes containing each of these proteins  in vitro.	bind
32046	1	9208	6	10	NULL	0	NULL	Bem1p	NULL		bind	NULL	directly			Cla4p	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7176_s_310	11113154	A Bem1p-dependent Complex Containing Cdc24p, Cdc42p, and Cla4p--  We report that Bem1p binds directly to Cla4p and to GTP-Cdc42p as well as to Cdc24p and can mediate the assembly of complexes containing each of these proteins  in vitro.	bind
32047	2	9208	6	10	NULL	0	NULL	Bem1p	NULL		bind	NULL	directly			GTP-Cdc42p	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7176_s_310	11113154	A Bem1p-dependent Complex Containing Cdc24p, Cdc42p, and Cla4p--  We report that Bem1p binds directly to Cla4p and to GTP-Cdc42p as well as to Cdc24p and can mediate the assembly of complexes containing each of these proteins  in vitro.	bind
32048	3	9208	6	10	NULL	0	NULL	Bem1p	NULL		bind	NULL	directly			Cdc24p	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7176_s_310	11113154	A Bem1p-dependent Complex Containing Cdc24p, Cdc42p, and Cla4p--  We report that Bem1p binds directly to Cla4p and to GTP-Cdc42p as well as to Cdc24p and can mediate the assembly of complexes containing each of these proteins  in vitro.	bind
32050	5	9208	6	10	NULL	0	NULL	Bem1p	NULL		mediate	NULL				Cla4p	NULL	assembly of complexes containing			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7176_s_310	11113154	A Bem1p-dependent Complex Containing Cdc24p, Cdc42p, and Cla4p--  We report that Bem1p binds directly to Cla4p and to GTP-Cdc42p as well as to Cdc24p and can mediate the assembly of complexes containing each of these proteins  in vitro.	bind
32051	6	9208	6	10	NULL	0	NULL	Bem1p	NULL		mediate	NULL				GTP-Cdc42p	NULL	assembly of complexes containing			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7176_s_310	11113154	A Bem1p-dependent Complex Containing Cdc24p, Cdc42p, and Cla4p--  We report that Bem1p binds directly to Cla4p and to GTP-Cdc42p as well as to Cdc24p and can mediate the assembly of complexes containing each of these proteins  in vitro.	bind
48053	4	9208	6	10	NULL	0	NULL	Bem1p			mediate					Cdc24p		assembly of complexes containing			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7176_s_310	11113154	A Bem1p-dependent Complex Containing Cdc24p, Cdc42p, and Cla4p--  We report that Bem1p binds directly to Cla4p and to GTP-Cdc42p as well as to Cdc24p and can mediate the assembly of complexes containing each of these proteins  in vitro.	bind
39647	1	9209	5	13	NULL	NULL	NULL	Bald	GP		is					benzaldehyde-activated transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_13_3926_s_7	12813087	A benzaldehyde-activated transcription factor (Bald) that specifically binds to the PAL  cis-acting element was also identified.	bind
39648	2	9209	5	13	NULL	NULL	NULL	Bald	GP		bind		specifically			PAL	GP			cis-acting element	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_13_3926_s_7	12813087	A benzaldehyde-activated transcription factor (Bald) that specifically binds to the PAL  cis-acting element was also identified.	bind
32052	1	9209	6	NULL	NULL	0	NULL	Bald	NULL		is	NULL				benzaldehyde-activated transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_185_13_3926_s_7	12813087	A benzaldehyde-activated transcription factor (Bald) that specifically binds to the PAL  cis-acting element was also identified.	bind
32053	2	9209	6	NULL	NULL	0	NULL	Bald	NULL		bind	NULL	specifically			PAL	NULL			cis-acting element	NULL		0	NULL	NULL	NULL	gw60_jbacteriol_185_13_3926_s_7	12813087	A benzaldehyde-activated transcription factor (Bald) that specifically binds to the PAL  cis-acting element was also identified.	bind
39649	1	9210	5	13	NULL	NULL	NULL	beta-cell-specific protein	GP		bind					B8	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4702_s_177	12052878	A beta-cell-specific protein binds to B8.	bind
32054	1	9210	6	NULL	NULL	0	NULL	beta-cell-specific protein	NULL		bind	NULL				B8	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_13_4702_s_177	12052878	A beta-cell-specific protein binds to B8.	bind
39650	1	9211	5	13	NULL	NULL	NULL	U1 RNA	NucleicAcid		bind					U1A protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_45_32265_s_24	10542265	A beta-sheet also plays a critical role in the binding of U1 RNA to the small nuclear ribonucleoprotein U1A protein ( 12).	bind
39651	2	9211	5	13	NULL	NULL	NULL	U1A protein	GP		is a type of					small nuclear ribonucleoprotein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_45_32265_s_24	10542265	A beta-sheet also plays a critical role in the binding of U1 RNA to the small nuclear ribonucleoprotein U1A protein ( 12).	bind
39652	3	9211	5	13	NULL	NULL	NULL	beta-sheet	GP		plays a role in		critical			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_45_32265_s_24	10542265	A beta-sheet also plays a critical role in the binding of U1 RNA to the small nuclear ribonucleoprotein U1A protein ( 12).	bind
32055	1	9211	6	10	NULL	0	NULL	U1 RNA	NULL		bind	NULL				 U1A protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_45_32265_s_24	10542265	A beta-sheet also plays a critical role in the binding of U1 RNA to the small nuclear ribonucleoprotein U1A protein ( 12).	bind
32056	2	9211	6	10	NULL	0	NULL	beta-sheet	NULL		plays a role in	NULL	critical			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_45_32265_s_24	10542265	A beta-sheet also plays a critical role in the binding of U1 RNA to the small nuclear ribonucleoprotein U1A protein ( 12).	bind
48054	3	9211	6	10	NULL	0	NULL	U1A protein	NULL		is a type of	NULL				small nuclear ribonucleoprotein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_45_32265_s_24	10542265	A beta-sheet also plays a critical role in the binding of U1 RNA to the small nuclear ribonucleoprotein U1A protein ( 12).	bind
40365	2	9214	5	13	NULL	NULL	NULL	beta4R1281W	GP		is					statement 1	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_3_1211_s_163	14668477	A beta4 subunit in which the binding site for the plectin-ABD is mutated (beta4R1281W) bound to plec1 - 606, plec284 - 1154, and plec1 - 1154.	bind
40366	3	9214	5	13	NULL	NULL	NULL				bind			beta4R1281W		plec	GP		1 - 606		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_3_1211_s_163	14668477	A beta4 subunit in which the binding site for the plectin-ABD is mutated (beta4R1281W) bound to plec1 - 606, plec284 - 1154, and plec1 - 1154.	bind
40367	5	9214	5	13	NULL	NULL	NULL				bind			beta4R1281W		plec	GP		284 - 1154		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_3_1211_s_163	14668477	A beta4 subunit in which the binding site for the plectin-ABD is mutated (beta4R1281W) bound to plec1 - 606, plec284 - 1154, and plec1 - 1154.	bind
40368	4	9214	5	13	NULL	NULL	NULL				bind			beta4R1281W		plec	GP		1 - 1154		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_3_1211_s_163	14668477	A beta4 subunit in which the binding site for the plectin-ABD is mutated (beta4R1281W) bound to plec1 - 606, plec284 - 1154, and plec1 - 1154.	bind
48055	1	9214	5	13	NULL	NULL	NULL	beta4 subunit	GP		contains								plectin-ABD binding site		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_3_1211_s_163	14668477	A beta4 subunit in which the binding site for the plectin-ABD is mutated (beta4R1281W) bound to plec1 - 606, plec284 - 1154, and plec1 - 1154.	bind
32069	1	9214	6	NULL	NULL	0	NULL	beta4 subunit	NULL	mutant	bind	NULL		plectin-ABD binding site		plec	NULL		1-606		NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_3_1211_s_163	14668477	A beta4 subunit in which the binding site for the plectin-ABD is mutated (beta4R1281W) bound to plec1 - 606, plec284 - 1154, and plec1 - 1154.	bind
32070	2	9214	6	NULL	NULL	0	NULL	beta4 subunit	NULL	mutant	bind	NULL		plectin-ABD binding site		plec	NULL		284-1154		NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_3_1211_s_163	14668477	A beta4 subunit in which the binding site for the plectin-ABD is mutated (beta4R1281W) bound to plec1 - 606, plec284 - 1154, and plec1 - 1154.	bind
32071	3	9214	6	NULL	NULL	0	NULL	beta4 subunit	NULL	mutant	bind	NULL		plectin-ABD binding site		plec	NULL		1-1154		NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_3_1211_s_163	14668477	A beta4 subunit in which the binding site for the plectin-ABD is mutated (beta4R1281W) bound to plec1 - 606, plec284 - 1154, and plec1 - 1154.	bind
48056	4	9214	6	10	NULL	0	NULL	beta4R1281W	NULL		is	NULL				beta4 subunit	NULL	mutant	 plectin-ABD binding site		NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_3_1211_s_163	14668477	A beta4 subunit in which the binding site for the plectin-ABD is mutated (beta4R1281W) bound to plec1 - 606, plec284 - 1154, and plec1 - 1154.	bind
39654	1	9215	5	13	NULL	NULL	NULL	SDF-1	GP		bind					CXCR4	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-clin-invest_115_1_15630439_s_3	15630439	A better understanding at a molecular level of how the binding of SDF-1  to its cell surface receptor, CXCR4, elicits specific biological responses  in these cells has now been achieved through the identification of PKC-zeta  activation as a common downstream signal.	bind
39655	2	9215	5	13	NULL	NULL	NULL	CXCR4	GP		is a type of					cell surface receptor	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-clin-invest_115_1_15630439_s_3	15630439	A better understanding at a molecular level of how the binding of SDF-1  to its cell surface receptor, CXCR4, elicits specific biological responses  in these cells has now been achieved through the identification of PKC-zeta  activation as a common downstream signal.	bind
39656	3	9215	5	13	NULL	NULL	NULL	statement 1	Process		elicits					biological responses	Process	specific			NULL	CXCR4	NULL	NULL	NULL	NULL	abs-batch0650-0679_j-clin-invest_115_1_15630439_s_3	15630439	A better understanding at a molecular level of how the binding of SDF-1  to its cell surface receptor, CXCR4, elicits specific biological responses  in these cells has now been achieved through the identification of PKC-zeta  activation as a common downstream signal.	bind
39657	4	9215	5	13	NULL	NULL	NULL	PKC-zeta	GP	activation of	acts as					downstream signal	Process	common			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-clin-invest_115_1_15630439_s_3	15630439	A better understanding at a molecular level of how the binding of SDF-1  to its cell surface receptor, CXCR4, elicits specific biological responses  in these cells has now been achieved through the identification of PKC-zeta  activation as a common downstream signal.	bind
39658	5	9215	5	13	NULL	NULL	NULL	statement 4	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-clin-invest_115_1_15630439_s_3	15630439	A better understanding at a molecular level of how the binding of SDF-1  to its cell surface receptor, CXCR4, elicits specific biological responses  in these cells has now been achieved through the identification of PKC-zeta  activation as a common downstream signal.	bind
32073	1	9215	6	NULL	NULL	0	NULL	SDF-1	NULL		bind	NULL				CXCR4	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-clin-invest_115_1_15630439_s_3	15630439	A better understanding at a molecular level of how the binding of SDF-1  to its cell surface receptor, CXCR4, elicits specific biological responses  in these cells has now been achieved through the identification of PKC-zeta  activation as a common downstream signal.	bind
32074	2	9215	6	NULL	NULL	0	NULL	CXCR4	NULL		is a type of	NULL				cell surface receptor	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-clin-invest_115_1_15630439_s_3	15630439	A better understanding at a molecular level of how the binding of SDF-1  to its cell surface receptor, CXCR4, elicits specific biological responses  in these cells has now been achieved through the identification of PKC-zeta  activation as a common downstream signal.	bind
32075	3	9215	6	10	NULL	0	NULL	statement 1			elicits					biological responses		specific			NULL	CXCR4	NULL	NULL	NULL	NULL	abs-batch0650-0679_j-clin-invest_115_1_15630439_s_3	15630439	A better understanding at a molecular level of how the binding of SDF-1  to its cell surface receptor, CXCR4, elicits specific biological responses  in these cells has now been achieved through the identification of PKC-zeta  activation as a common downstream signal.	bind
57855	4	9215	6	10	NULL	0	NULL	PKC-zeta		activation of	acts as					downstream signal		common			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-clin-invest_115_1_15630439_s_3	15630439	A better understanding at a molecular level of how the binding of SDF-1  to its cell surface receptor, CXCR4, elicits specific biological responses  in these cells has now been achieved through the identification of PKC-zeta  activation as a common downstream signal.	bind
57856	5	9215	6	10	NULL	0	NULL	statement 4			leads to					statement 3					NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-clin-invest_115_1_15630439_s_3	15630439	A better understanding at a molecular level of how the binding of SDF-1  to its cell surface receptor, CXCR4, elicits specific biological responses  in these cells has now been achieved through the identification of PKC-zeta  activation as a common downstream signal.	bind
39659	1	9216	5	13	NULL	NULL	NULL	GTF3	GP		bind			R4		DNA sequence	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_31722_s_296	15987678	A better understanding of the involvement of this area in DNA-protein interaction will require knowledge of the crystal structure of GTF3-R4 bound to its target DNA sequence.	bind
32076	1	9216	6	NULL	NULL	0	NULL	GTF3	NULL		bind	NULL		R4		DNA sequence	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_36_31722_s_296	15987678	A better understanding of the involvement of this area in DNA-protein interaction will require knowledge of the crystal structure of GTF3-R4 bound to its target DNA sequence.	bind
39660	1	9217	5	13	NULL	NULL	NULL	PAM2	GP		bind					HYD	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_20_14376_s_48	16554297	A better understanding of the PAM2 binding properties of HYD should help elucidate its function through identification of novel physiological partners and provide useful insight into the potential competition between HYD and PABP for shared binding partners.	bind
32077	1	9217	6	NULL	NULL	0	NULL	HYD	NULL		bind	NULL				PAM2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_20_14376_s_48	16554297	A better understanding of the PAM2 binding properties of HYD should help elucidate its function through identification of novel physiological partners and provide useful insight into the potential competition between HYD and PABP for shared binding partners.	bind
39661	1	9218	5	13	NULL	NULL	NULL	CD46	GP		bind					MVH	GP	soluble			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_35_32294_s_137	12065582	A BIAcore 2000 instrument was used to monitor CD46 binding to soluble MVH.	bind
32078	1	9218	6	NULL	NULL	0	NULL	CD46	NULL		bind	NULL				MVH	NULL	soluble			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_35_32294_s_137	12065582	A BIAcore 2000 instrument was used to monitor CD46 binding to soluble MVH.	bind
39662	1	9219	5	13	NULL	NULL	NULL	IL-1 ligands	GP		bind					T1/ST2 Fc	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_10_5784_s_29	8621446	A BIAcore biosensor  (Pharmacia Biosensor) was used to examine binding of IL-1 ligands to  the human T1/ST2 Fc fusion protein, essentially as described in detail  in Arend  et al.( 14 ) .	bind
48057	2	9219	5	13	NULL	NULL	NULL	T1/ST2 Fc	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_10_5784_s_29	8621446	A BIAcore biosensor  (Pharmacia Biosensor) was used to examine binding of IL-1 ligands to  the human T1/ST2 Fc fusion protein, essentially as described in detail  in Arend  et al.( 14 ) .	bind
32099	1	9219	6	10	NULL	0	NULL	IL-1 ligands	NULL		bind	NULL				T1/ST2 Fc 	NULL	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_10_5784_s_29	8621446	A BIAcore biosensor  (Pharmacia Biosensor) was used to examine binding of IL-1 ligands to  the human T1/ST2 Fc fusion protein, essentially as described in detail  in Arend  et al.( 14 ) .	bind
48058	2	9219	6	10	NULL	0	NULL	T1/ST2 Fc	NULL		is a type of	NULL				fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_10_5784_s_29	8621446	A BIAcore biosensor  (Pharmacia Biosensor) was used to examine binding of IL-1 ligands to  the human T1/ST2 Fc fusion protein, essentially as described in detail  in Arend  et al.( 14 ) .	bind
39663	1	9220	5	13	NULL	NULL	NULL	BirA	GP		is a type of					bifunctional protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13513_s_360	16533810	A bifunctional protein (BirA) acts as a protein-biotin ligase or as a sensor-like transcriptional regulator ( ), and after complexation of BirA with biotin-5''-AMP ( ) or with biotin ( ), BirA monomers bind cooperatively to the biotin operator.	bind
39664	2	9220	5	13	NULL	NULL	NULL	BirA	GP		acts as					protein-biotin ligase	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13513_s_360	16533810	A bifunctional protein (BirA) acts as a protein-biotin ligase or as a sensor-like transcriptional regulator ( ), and after complexation of BirA with biotin-5''-AMP ( ) or with biotin ( ), BirA monomers bind cooperatively to the biotin operator.	bind
39665	3	9220	5	13	NULL	NULL	NULL	BirA	GP		acts as					sensor-like transcriptional regulator	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13513_s_360	16533810	A bifunctional protein (BirA) acts as a protein-biotin ligase or as a sensor-like transcriptional regulator ( ), and after complexation of BirA with biotin-5''-AMP ( ) or with biotin ( ), BirA monomers bind cooperatively to the biotin operator.	bind
39666	4	9220	5	13	NULL	NULL	NULL	BirA	GP		complex with					biotin-5''-AMP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13513_s_360	16533810	A bifunctional protein (BirA) acts as a protein-biotin ligase or as a sensor-like transcriptional regulator ( ), and after complexation of BirA with biotin-5''-AMP ( ) or with biotin ( ), BirA monomers bind cooperatively to the biotin operator.	bind
39667	5	9220	5	13	NULL	NULL	NULL	BirA	GP		complex with					biotin	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13513_s_360	16533810	A bifunctional protein (BirA) acts as a protein-biotin ligase or as a sensor-like transcriptional regulator ( ), and after complexation of BirA with biotin-5''-AMP ( ) or with biotin ( ), BirA monomers bind cooperatively to the biotin operator.	bind
39668	6	9220	5	13	NULL	NULL	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13513_s_360	16533810	A bifunctional protein (BirA) acts as a protein-biotin ligase or as a sensor-like transcriptional regulator ( ), and after complexation of BirA with biotin-5''-AMP ( ) or with biotin ( ), BirA monomers bind cooperatively to the biotin operator.	bind
39669	7	9220	5	13	NULL	NULL	NULL	BirA monomers	GP		bind		cooperatively			biotin	Chemical			operator	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13513_s_360	16533810	A bifunctional protein (BirA) acts as a protein-biotin ligase or as a sensor-like transcriptional regulator ( ), and after complexation of BirA with biotin-5''-AMP ( ) or with biotin ( ), BirA monomers bind cooperatively to the biotin operator.	bind
39670	8	9220	5	13	NULL	NULL	NULL	statement 7	Process		occurs after					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13513_s_360	16533810	A bifunctional protein (BirA) acts as a protein-biotin ligase or as a sensor-like transcriptional regulator ( ), and after complexation of BirA with biotin-5''-AMP ( ) or with biotin ( ), BirA monomers bind cooperatively to the biotin operator.	bind
39671	9	9220	5	13	NULL	NULL	NULL	statement 7	Process		occurs after					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13513_s_360	16533810	A bifunctional protein (BirA) acts as a protein-biotin ligase or as a sensor-like transcriptional regulator ( ), and after complexation of BirA with biotin-5''-AMP ( ) or with biotin ( ), BirA monomers bind cooperatively to the biotin operator.	bind
32101	1	9220	6	NULL	NULL	0	NULL	BirA	NULL		is a type of	NULL				bifunctional protein	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_19_13513_s_360	16533810	A bifunctional protein (BirA) acts as a protein-biotin ligase or as a sensor-like transcriptional regulator ( ), and after complexation of BirA with biotin-5''-AMP ( ) or with biotin ( ), BirA monomers bind cooperatively to the biotin operator.	bind
32102	2	9220	6	NULL	NULL	0	NULL	BirA	NULL		functions as a	NULL				protein-biotin ligase	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_19_13513_s_360	16533810	A bifunctional protein (BirA) acts as a protein-biotin ligase or as a sensor-like transcriptional regulator ( ), and after complexation of BirA with biotin-5''-AMP ( ) or with biotin ( ), BirA monomers bind cooperatively to the biotin operator.	bind
32103	3	9220	6	10	NULL	0	NULL	BirA			functions as a					sensor like transcriptional regulator					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13513_s_360	16533810	A bifunctional protein (BirA) acts as a protein-biotin ligase or as a sensor-like transcriptional regulator ( ), and after complexation of BirA with biotin-5''-AMP ( ) or with biotin ( ), BirA monomers bind cooperatively to the biotin operator.	bind
32106	4	9220	6	NULL	NULL	0	NULL	BirA	NULL		complexes with	NULL				biotin-5''-AMP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_19_13513_s_360	16533810	A bifunctional protein (BirA) acts as a protein-biotin ligase or as a sensor-like transcriptional regulator ( ), and after complexation of BirA with biotin-5''-AMP ( ) or with biotin ( ), BirA monomers bind cooperatively to the biotin operator.	bind
32109	5	9220	6	NULL	NULL	0	NULL	BirA	NULL		complexes with	NULL				biotin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_19_13513_s_360	16533810	A bifunctional protein (BirA) acts as a protein-biotin ligase or as a sensor-like transcriptional regulator ( ), and after complexation of BirA with biotin-5''-AMP ( ) or with biotin ( ), BirA monomers bind cooperatively to the biotin operator.	bind
32110	6	9220	6	NULL	NULL	0	NULL	BirA monomers	NULL		bind	NULL	cooperatively			biotin	NULL			operator	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_19_13513_s_360	16533810	A bifunctional protein (BirA) acts as a protein-biotin ligase or as a sensor-like transcriptional regulator ( ), and after complexation of BirA with biotin-5''-AMP ( ) or with biotin ( ), BirA monomers bind cooperatively to the biotin operator.	bind
32111	7	9220	6	NULL	NULL	0	NULL	statement 6	NULL		occurs after	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_19_13513_s_360	16533810	A bifunctional protein (BirA) acts as a protein-biotin ligase or as a sensor-like transcriptional regulator ( ), and after complexation of BirA with biotin-5''-AMP ( ) or with biotin ( ), BirA monomers bind cooperatively to the biotin operator.	bind
32112	8	9220	6	NULL	NULL	0	NULL	statement 6	NULL		occurs after	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_19_13513_s_360	16533810	A bifunctional protein (BirA) acts as a protein-biotin ligase or as a sensor-like transcriptional regulator ( ), and after complexation of BirA with biotin-5''-AMP ( ) or with biotin ( ), BirA monomers bind cooperatively to the biotin operator.	bind
57857	9	9220	6	10	NULL	0	NULL	statement 4			is an alternative to					statement 5					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_19_13513_s_360	16533810	A bifunctional protein (BirA) acts as a protein-biotin ligase or as a sensor-like transcriptional regulator ( ), and after complexation of BirA with biotin-5''-AMP ( ) or with biotin ( ), BirA monomers bind cooperatively to the biotin operator.	bind
39672	1	9221	5	13	NULL	NULL	NULL	Bim BH3 peptide	GP		interact with		potentially			anti-apoptotic proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_9_5750_s_286	16380381	A Bim BH3 peptide appears capable of interacting with most anti-apoptotic proteins including Mcl-1 with high affinity, whereas the Bid BH3 peptide does not bind Mcl-1.	bind
39673	2	9221	5	13	NULL	NULL	NULL	Mcl-1	GP		is a type of					anti-apoptotic proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_9_5750_s_286	16380381	A Bim BH3 peptide appears capable of interacting with most anti-apoptotic proteins including Mcl-1 with high affinity, whereas the Bid BH3 peptide does not bind Mcl-1.	bind
39674	3	9221	5	13	NULL	NULL	NULL	Bim BH3 peptide	GP		interact with		high affinity			Mcl-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_9_5750_s_286	16380381	A Bim BH3 peptide appears capable of interacting with most anti-apoptotic proteins including Mcl-1 with high affinity, whereas the Bid BH3 peptide does not bind Mcl-1.	bind
39675	4	9221	5	13	NULL	NULL	NULL	Bid BH3 peptide	GP		does not bind					Mcl-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_9_5750_s_286	16380381	A Bim BH3 peptide appears capable of interacting with most anti-apoptotic proteins including Mcl-1 with high affinity, whereas the Bid BH3 peptide does not bind Mcl-1.	bind
32238	1	9221	6	10	NULL	0	NULL	Bim BH3 peptide			interacts with		high affinity			Mcl-1					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_9_5750_s_286	16380381	A Bim BH3 peptide appears capable of interacting with most anti-apoptotic proteins including Mcl-1 with high affinity, whereas the Bid BH3 peptide does not bind Mcl-1.	bind
32239	2	9221	6	NULL	NULL	0	NULL	Mcl-1	NULL		is a type of	NULL				anti-apoptotic protein	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_9_5750_s_286	16380381	A Bim BH3 peptide appears capable of interacting with most anti-apoptotic proteins including Mcl-1 with high affinity, whereas the Bid BH3 peptide does not bind Mcl-1.	bind
32240	3	9221	6	NULL	NULL	0	NULL	Bid BH3 peptide	NULL		does not bind	NULL				Mcl-1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_9_5750_s_286	16380381	A Bim BH3 peptide appears capable of interacting with most anti-apoptotic proteins including Mcl-1 with high affinity, whereas the Bid BH3 peptide does not bind Mcl-1.	bind
39676	1	9222	5	13	NULL	NULL	NULL	Fos kinase	GP		bind					BIM	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_6_3385_s_145	9920881	A BIM-insensitive Fos peptide kinase eluting at 70 mM NaCl (fraction 18) was used as a negative control to test the specific nature of Fos kinase binding to the BIM-Sepharose.	bind
48059	1	9222	6	10	NULL	0	NULL	Fos kinase	NULL		bind	NULL				BIM	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_6_3385_s_145	9920881	A BIM-insensitive Fos peptide kinase eluting at 70 mM NaCl (fraction 18) was used as a negative control to test the specific nature of Fos kinase binding to the BIM-Sepharose.	bind
39677	1	9223	5	13	NULL	NULL	NULL	BRG1	GP	purified;;E.coli-expressed;;histidine-tagged	bind		directly	295 - 634		HP1alpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_21_5797_s_81	12411497	A binding assay carried out with a purified  E.coli-expressed histidine-tagged BRG1 fragment bearing residues 295 - 634 [referred to here as His-BRG1(295 - 634) in Figure  4] demonstrated direct binding to HP1alpha (lane 3), but not to HP1beta (lane 5) and HP1gamma (lane 7), whereas, under similar conditions, purified calf thymus histone H3 and recombinant TIF1beta bound to all three GST - HP1s (Figure  4F and data not shown).	bind
39678	2	9223	5	13	NULL	NULL	NULL	BRG1	GP	purified;;E.coli-expressed;;histidine-tagged	does not bind			295 - 634		HP1beta	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_21_5797_s_81	12411497	A binding assay carried out with a purified  E.coli-expressed histidine-tagged BRG1 fragment bearing residues 295 - 634 [referred to here as His-BRG1(295 - 634) in Figure  4] demonstrated direct binding to HP1alpha (lane 3), but not to HP1beta (lane 5) and HP1gamma (lane 7), whereas, under similar conditions, purified calf thymus histone H3 and recombinant TIF1beta bound to all three GST - HP1s (Figure  4F and data not shown).	bind
39679	3	9223	5	13	NULL	NULL	NULL	BRG1	GP	purified;;E.coli-expressed;;histidine-tagged	does not bind			295 - 634		HP1gamma	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_21_5797_s_81	12411497	A binding assay carried out with a purified  E.coli-expressed histidine-tagged BRG1 fragment bearing residues 295 - 634 [referred to here as His-BRG1(295 - 634) in Figure  4] demonstrated direct binding to HP1alpha (lane 3), but not to HP1beta (lane 5) and HP1gamma (lane 7), whereas, under similar conditions, purified calf thymus histone H3 and recombinant TIF1beta bound to all three GST - HP1s (Figure  4F and data not shown).	bind
39680	4	9223	5	13	NULL	NULL	NULL	H3	GP		is a type of					histone	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_21_5797_s_81	12411497	A binding assay carried out with a purified  E.coli-expressed histidine-tagged BRG1 fragment bearing residues 295 - 634 [referred to here as His-BRG1(295 - 634) in Figure  4] demonstrated direct binding to HP1alpha (lane 3), but not to HP1beta (lane 5) and HP1gamma (lane 7), whereas, under similar conditions, purified calf thymus histone H3 and recombinant TIF1beta bound to all three GST - HP1s (Figure  4F and data not shown).	bind
39681	5	9223	5	13	NULL	NULL	NULL	H3	GP	purified;;calf thymus	bind					GST - HP1alpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_21_5797_s_81	12411497	A binding assay carried out with a purified  E.coli-expressed histidine-tagged BRG1 fragment bearing residues 295 - 634 [referred to here as His-BRG1(295 - 634) in Figure  4] demonstrated direct binding to HP1alpha (lane 3), but not to HP1beta (lane 5) and HP1gamma (lane 7), whereas, under similar conditions, purified calf thymus histone H3 and recombinant TIF1beta bound to all three GST - HP1s (Figure  4F and data not shown).	bind
39682	6	9223	5	13	NULL	NULL	NULL	H3	GP	purified;;calf thymus	bind					GST - HP1beta	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_21_5797_s_81	12411497	A binding assay carried out with a purified  E.coli-expressed histidine-tagged BRG1 fragment bearing residues 295 - 634 [referred to here as His-BRG1(295 - 634) in Figure  4] demonstrated direct binding to HP1alpha (lane 3), but not to HP1beta (lane 5) and HP1gamma (lane 7), whereas, under similar conditions, purified calf thymus histone H3 and recombinant TIF1beta bound to all three GST - HP1s (Figure  4F and data not shown).	bind
39683	7	9223	5	13	NULL	NULL	NULL	H3	GP	purified;;calf thymus	bind					GST - HP1gamma	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_21_5797_s_81	12411497	A binding assay carried out with a purified  E.coli-expressed histidine-tagged BRG1 fragment bearing residues 295 - 634 [referred to here as His-BRG1(295 - 634) in Figure  4] demonstrated direct binding to HP1alpha (lane 3), but not to HP1beta (lane 5) and HP1gamma (lane 7), whereas, under similar conditions, purified calf thymus histone H3 and recombinant TIF1beta bound to all three GST - HP1s (Figure  4F and data not shown).	bind
39684	8	9223	5	13	NULL	NULL	NULL	TIF1beta	GP	recombinant	bind					GST - HP1alpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_21_5797_s_81	12411497	A binding assay carried out with a purified  E.coli-expressed histidine-tagged BRG1 fragment bearing residues 295 - 634 [referred to here as His-BRG1(295 - 634) in Figure  4] demonstrated direct binding to HP1alpha (lane 3), but not to HP1beta (lane 5) and HP1gamma (lane 7), whereas, under similar conditions, purified calf thymus histone H3 and recombinant TIF1beta bound to all three GST - HP1s (Figure  4F and data not shown).	bind
39685	9	9223	5	13	NULL	NULL	NULL	TIF1beta	GP	recombinant	bind					GST - HP1beta	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_21_5797_s_81	12411497	A binding assay carried out with a purified  E.coli-expressed histidine-tagged BRG1 fragment bearing residues 295 - 634 [referred to here as His-BRG1(295 - 634) in Figure  4] demonstrated direct binding to HP1alpha (lane 3), but not to HP1beta (lane 5) and HP1gamma (lane 7), whereas, under similar conditions, purified calf thymus histone H3 and recombinant TIF1beta bound to all three GST - HP1s (Figure  4F and data not shown).	bind
39686	10	9223	5	13	NULL	NULL	NULL	TIF1beta	GP	recombinant	bind					GST - HP1gamma	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_21_5797_s_81	12411497	A binding assay carried out with a purified  E.coli-expressed histidine-tagged BRG1 fragment bearing residues 295 - 634 [referred to here as His-BRG1(295 - 634) in Figure  4] demonstrated direct binding to HP1alpha (lane 3), but not to HP1beta (lane 5) and HP1gamma (lane 7), whereas, under similar conditions, purified calf thymus histone H3 and recombinant TIF1beta bound to all three GST - HP1s (Figure  4F and data not shown).	bind
32548	1	9223	6	NULL	NULL	0	NULL	His-BRG1	NULL		bind	NULL	directly	295-634		Hp1alpha	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_21_21_5797_s_81	12411497	A binding assay carried out with a purified  E.coli-expressed histidine-tagged BRG1 fragment bearing residues 295 - 634 [referred to here as His-BRG1(295 - 634) in Figure  4] demonstrated direct binding to HP1alpha (lane 3), but not to HP1beta (lane 5) and HP1gamma (lane 7), whereas, under similar conditions, purified calf thymus histone H3 and recombinant TIF1beta bound to all three GST - HP1s (Figure  4F and data not shown).	bind
32550	2	9223	6	10	NULL	0	NULL	His-BRG1	NULL		is	NULL				BRG1 fragment	NULL	purified;; E.coli-expressed;; histidine tagged			NULL		NULL	NULL	NULL	NULL	gw60_embo_21_21_5797_s_81	12411497	A binding assay carried out with a purified  E.coli-expressed histidine-tagged BRG1 fragment bearing residues 295 - 634 [referred to here as His-BRG1(295 - 634) in Figure  4] demonstrated direct binding to HP1alpha (lane 3), but not to HP1beta (lane 5) and HP1gamma (lane 7), whereas, under similar conditions, purified calf thymus histone H3 and recombinant TIF1beta bound to all three GST - HP1s (Figure  4F and data not shown).	bind
32551	3	9223	6	NULL	NULL	0	NULL	His-BRG1	NULL		does not bind	NULL		295-634		HP1gamma	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_21_21_5797_s_81	12411497	A binding assay carried out with a purified  E.coli-expressed histidine-tagged BRG1 fragment bearing residues 295 - 634 [referred to here as His-BRG1(295 - 634) in Figure  4] demonstrated direct binding to HP1alpha (lane 3), but not to HP1beta (lane 5) and HP1gamma (lane 7), whereas, under similar conditions, purified calf thymus histone H3 and recombinant TIF1beta bound to all three GST - HP1s (Figure  4F and data not shown).	bind
32552	4	9223	6	10	NULL	0	NULL	 H3		purified;; calf thymus	bind					GST-HP1alpha					NULL		NULL	NULL	NULL	NULL	gw60_embo_21_21_5797_s_81	12411497	A binding assay carried out with a purified  E.coli-expressed histidine-tagged BRG1 fragment bearing residues 295 - 634 [referred to here as His-BRG1(295 - 634) in Figure  4] demonstrated direct binding to HP1alpha (lane 3), but not to HP1beta (lane 5) and HP1gamma (lane 7), whereas, under similar conditions, purified calf thymus histone H3 and recombinant TIF1beta bound to all three GST - HP1s (Figure  4F and data not shown).	bind
32553	5	9223	6	10	NULL	0	NULL	TIF1beta	NULL	recombinant	bind	NULL				GST-HP1alpha	NULL				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_21_5797_s_81	12411497	A binding assay carried out with a purified  E.coli-expressed histidine-tagged BRG1 fragment bearing residues 295 - 634 [referred to here as His-BRG1(295 - 634) in Figure  4] demonstrated direct binding to HP1alpha (lane 3), but not to HP1beta (lane 5) and HP1gamma (lane 7), whereas, under similar conditions, purified calf thymus histone H3 and recombinant TIF1beta bound to all three GST - HP1s (Figure  4F and data not shown).	bind
48060	6	9223	6	10	NULL	0	NULL	His-BRG1	NULL		does not bind	NULL		295 - 634		HP1beta	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_21_21_5797_s_81	12411497	A binding assay carried out with a purified  E.coli-expressed histidine-tagged BRG1 fragment bearing residues 295 - 634 [referred to here as His-BRG1(295 - 634) in Figure  4] demonstrated direct binding to HP1alpha (lane 3), but not to HP1beta (lane 5) and HP1gamma (lane 7), whereas, under similar conditions, purified calf thymus histone H3 and recombinant TIF1beta bound to all three GST - HP1s (Figure  4F and data not shown).	bind
48061	7	9223	6	10	NULL	0	NULL	 H3		purified;; calf thymus	bind					GST-HP1beta					NULL		NULL	NULL	NULL	NULL	gw60_embo_21_21_5797_s_81	12411497	A binding assay carried out with a purified  E.coli-expressed histidine-tagged BRG1 fragment bearing residues 295 - 634 [referred to here as His-BRG1(295 - 634) in Figure  4] demonstrated direct binding to HP1alpha (lane 3), but not to HP1beta (lane 5) and HP1gamma (lane 7), whereas, under similar conditions, purified calf thymus histone H3 and recombinant TIF1beta bound to all three GST - HP1s (Figure  4F and data not shown).	bind
48062	8	9223	6	10	NULL	0	NULL	 H3		purified;; calf thymus	bind					GST-HP1gamma					NULL		NULL	NULL	NULL	NULL	gw60_embo_21_21_5797_s_81	12411497	A binding assay carried out with a purified  E.coli-expressed histidine-tagged BRG1 fragment bearing residues 295 - 634 [referred to here as His-BRG1(295 - 634) in Figure  4] demonstrated direct binding to HP1alpha (lane 3), but not to HP1beta (lane 5) and HP1gamma (lane 7), whereas, under similar conditions, purified calf thymus histone H3 and recombinant TIF1beta bound to all three GST - HP1s (Figure  4F and data not shown).	bind
48063	9	9223	6	10	NULL	0	NULL	TIF1beta 	NULL	recombinant	bind	NULL				GST-HP1beta	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_21_21_5797_s_81	12411497	A binding assay carried out with a purified  E.coli-expressed histidine-tagged BRG1 fragment bearing residues 295 - 634 [referred to here as His-BRG1(295 - 634) in Figure  4] demonstrated direct binding to HP1alpha (lane 3), but not to HP1beta (lane 5) and HP1gamma (lane 7), whereas, under similar conditions, purified calf thymus histone H3 and recombinant TIF1beta bound to all three GST - HP1s (Figure  4F and data not shown).	bind
48064	10	9223	6	10	NULL	0	NULL	TIF1beta 	NULL	recombinant	bind	NULL				GST-HP1gamma	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_21_21_5797_s_81	12411497	A binding assay carried out with a purified  E.coli-expressed histidine-tagged BRG1 fragment bearing residues 295 - 634 [referred to here as His-BRG1(295 - 634) in Figure  4] demonstrated direct binding to HP1alpha (lane 3), but not to HP1beta (lane 5) and HP1gamma (lane 7), whereas, under similar conditions, purified calf thymus histone H3 and recombinant TIF1beta bound to all three GST - HP1s (Figure  4F and data not shown).	bind
57858	11	9223	6	10	NULL	0	NULL	H3			is a type of					histone					NULL		0	NULL	NULL	NULL	gw60_embo_21_21_5797_s_81	12411497	A binding assay carried out with a purified  E.coli-expressed histidine-tagged BRG1 fragment bearing residues 295 - 634 [referred to here as His-BRG1(295 - 634) in Figure  4] demonstrated direct binding to HP1alpha (lane 3), but not to HP1beta (lane 5) and HP1gamma (lane 7), whereas, under similar conditions, purified calf thymus histone H3 and recombinant TIF1beta bound to all three GST - HP1s (Figure  4F and data not shown).	bind
39687	1	9224	5	13	NULL	NULL	NULL	GBR 12935	Chemical		bind					striatal membranes	CellComponent	rat			NULL		NULL	NULL	NULL	NULL	gw60_brainres_981_1_85_s_43	12885429	A binding assay for the DA uptake complex using [3]GBR 12935 binding to rat striatal membranes was conducted as per Anderson [  1.	bind
32241	1	9224	6	NULL	NULL	0	NULL	GBR 12935	NULL		bind	NULL				striatal membranes	NULL	rat			NULL		0	NULL	NULL	NULL	gw60_brainres_981_1_85_s_43	12885429	A binding assay for the DA uptake complex using [3]GBR 12935 binding to rat striatal membranes was conducted as per Anderson [  1.	bind
39688	1	9225	5	13	NULL	NULL	NULL	A1B	NucleicAcid	recombinant	bind		specifically			CE1d	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_33_29745_s_203	12060656	A binding assay performed with recombinant A1B also indicated specific binding to CE1d (Fig.  5 D,  top right panel) and stronger binding to M7* relative to M6* RNA ( bottom right panel).	bind
39689	2	9225	5	13	NULL	NULL	NULL	A1B	NucleicAcid	recombinant	bind					M7* RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_33_29745_s_203	12060656	A binding assay performed with recombinant A1B also indicated specific binding to CE1d (Fig.  5 D,  top right panel) and stronger binding to M7* relative to M6* RNA ( bottom right panel).	bind
39690	3	9225	5	13	NULL	NULL	NULL	A1B	NucleicAcid	recombinant	bind					M6* RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_33_29745_s_203	12060656	A binding assay performed with recombinant A1B also indicated specific binding to CE1d (Fig.  5 D,  top right panel) and stronger binding to M7* relative to M6* RNA ( bottom right panel).	bind
39691	4	9225	5	13	NULL	NULL	NULL	statement 2	Process		is stronger than					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_33_29745_s_203	12060656	A binding assay performed with recombinant A1B also indicated specific binding to CE1d (Fig.  5 D,  top right panel) and stronger binding to M7* relative to M6* RNA ( bottom right panel).	bind
32242	1	9225	6	NULL	NULL	0	NULL	A1B	NULL	recombinant	bind	NULL	specifically			CE1d	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_33_29745_s_203	12060656	A binding assay performed with recombinant A1B also indicated specific binding to CE1d (Fig.  5 D,  top right panel) and stronger binding to M7* relative to M6* RNA ( bottom right panel).	bind
32243	2	9225	6	10	NULL	0	NULL	A1B		recombinant	bind					M7* RNA					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_33_29745_s_203	12060656	A binding assay performed with recombinant A1B also indicated specific binding to CE1d (Fig.  5 D,  top right panel) and stronger binding to M7* relative to M6* RNA ( bottom right panel).	bind
32244	3	9225	6	10	NULL	0	NULL	A1B		recombinant	bind					M6* RNA					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_33_29745_s_203	12060656	A binding assay performed with recombinant A1B also indicated specific binding to CE1d (Fig.  5 D,  top right panel) and stronger binding to M7* relative to M6* RNA ( bottom right panel).	bind
32245	4	9225	6	NULL	NULL	0	NULL	statement 2	NULL	affinity of	is greater than	NULL				statement 3	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_33_29745_s_203	12060656	A binding assay performed with recombinant A1B also indicated specific binding to CE1d (Fig.  5 D,  top right panel) and stronger binding to M7* relative to M6* RNA ( bottom right panel).	bind
39692	1	9226	5	13	NULL	NULL	NULL	vimentin	GP		bind			tail		F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_41_30393_s_173	16901892	A binding assay showed that the vimentin tail binds F-actin with a  Kd of  14 muM.	bind
32246	1	9226	6	10	NULL	0	NULL	vimentin 	NULL		bind	NULL		tail		F-actin	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_41_30393_s_173	16901892	A binding assay showed that the vimentin tail binds F-actin with a  Kd of  14 muM.	bind
39693	1	9227	5	13	NULL	NULL	NULL	CCL3	GP		bind					CCR1	GP				NULL	CCR1-transfected HEK 293 cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_42_40473_s_96	12909630	A binding assay using CCR1-transfected HEK 293 cells was used to screen our compound library for small molecular weight compounds that inhibit CCL3 binding to CCR1.	bind
39694	2	9227	5	13	NULL	NULL	NULL	small molecular weight compounds	Chemical		inhibit					statement 1	Process				NULL	CCR1-transfected HEK 293 cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_42_40473_s_96	12909630	A binding assay using CCR1-transfected HEK 293 cells was used to screen our compound library for small molecular weight compounds that inhibit CCL3 binding to CCR1.	bind
32247	1	9227	6	10	NULL	0	NULL	CCL3	NULL		bind	NULL				CCR1	NULL				NULL	CCR1-transfected HEK 293 cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_42_40473_s_96	12909630	A binding assay using CCR1-transfected HEK 293 cells was used to screen our compound library for small molecular weight compounds that inhibit CCL3 binding to CCR1.	bind
48065	2	9227	6	10	NULL	0	NULL	small molecular weight compounds	NULL		inhibit	NULL				statement 1	NULL				NULL	CCR1-transfected HEK 293 cells	0	NULL	NULL	NULL	gw70_jbiolchem_278_42_40473_s_96	12909630	A binding assay using CCR1-transfected HEK 293 cells was used to screen our compound library for small molecular weight compounds that inhibit CCL3 binding to CCR1.	bind
39695	1	9228	5	13	NULL	NULL	NULL	SecE	GP		bind		may	C2		SecY	GP		C4		NULL		NULL	NULL	NULL	NULL	gw60_febslett_408_1_11_s_17	9180258	A binding between C2 of SecE and C4 of SecY may thus be suggested.	bind
32248	1	9228	6	NULL	NULL	0	NULL	SecE	NULL		bind	NULL	may	C2		SecY	NULL		C4		NULL		0	NULL	NULL	NULL	gw60_febslett_408_1_11_s_17	9180258	A binding between C2 of SecE and C4 of SecY may thus be suggested.	bind
40369	1	9229	5	13	NULL	NULL	NULL			wild-type;;human	does not complex with				betaA/-rich element	UL	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_15_5143_s_241	12861002	A binding complex did not form when the wild-type human betaA/-rich element was reacted with UL, whereas a specific binding complex formed when in vitro-synthesized RTEF-1b was added to binding reaction mixtures (Fig.  3B, lane 16 versus 17).	bind
32249	1	9229	6	NULL	NULL	0	NULL		NULL	wild type;; human	does not form a complex with	NULL			betaA/-rich element	UL	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_15_5143_s_241	12861002	A binding complex did not form when the wild-type human betaA/-rich element was reacted with UL, whereas a specific binding complex formed when in vitro-synthesized RTEF-1b was added to binding reaction mixtures (Fig.  3B, lane 16 versus 17).	bind
40373	3	9230	5	13	NULL	NULL	NULL	statement 1	GP		bind					B8 binding complex	GP	beta-cell-enriched			NULL	unfractionated betaTC-3 nuclear extract	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4702_s_183	12052878	A binding complex was detected in fractions 6 (44-kDa lower limit) and 7 (58-kDa upper limit) that comigrated with the beta-cell-enriched B8 binding complex in unfractionated betaTC-3 nuclear extract.	bind
40374	1	9230	5	13	NULL	NULL	NULL	binding complex	GP		is present in					44-kDa fraction	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4702_s_183	12052878	A binding complex was detected in fractions 6 (44-kDa lower limit) and 7 (58-kDa upper limit) that comigrated with the beta-cell-enriched B8 binding complex in unfractionated betaTC-3 nuclear extract.	bind
40375	2	9230	5	13	NULL	NULL	NULL	binding complex	GP		is present in					58-kDa fraction	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4702_s_183	12052878	A binding complex was detected in fractions 6 (44-kDa lower limit) and 7 (58-kDa upper limit) that comigrated with the beta-cell-enriched B8 binding complex in unfractionated betaTC-3 nuclear extract.	bind
40376	4	9230	5	13	NULL	NULL	NULL	statement 2	GP		bind					B8 binding complex	GP	beta-cell-enriched			NULL	unfractionated betaTC-3 nuclear extract	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4702_s_183	12052878	A binding complex was detected in fractions 6 (44-kDa lower limit) and 7 (58-kDa upper limit) that comigrated with the beta-cell-enriched B8 binding complex in unfractionated betaTC-3 nuclear extract.	bind
48066	1	9230	6	10	NULL	0	NULL	44-kDa protein	NULL		bind	NULL				 B8 binding complex	NULL	beta-cell-enriched			NULL	unfractionated betaTC-3 nuclear extract	0	NULL	NULL	NULL	gw60_molcellbiol_22_13_4702_s_183	12052878	A binding complex was detected in fractions 6 (44-kDa lower limit) and 7 (58-kDa upper limit) that comigrated with the beta-cell-enriched B8 binding complex in unfractionated betaTC-3 nuclear extract.	bind
48067	2	9230	6	10	NULL	0	NULL	58-kDa protein	NULL		bind	NULL				B8 binding complex	NULL	beta-cell-enriched			NULL	unfractionated betaTC-3 nuclear extract	0	NULL	NULL	NULL	gw60_molcellbiol_22_13_4702_s_183	12052878	A binding complex was detected in fractions 6 (44-kDa lower limit) and 7 (58-kDa upper limit) that comigrated with the beta-cell-enriched B8 binding complex in unfractionated betaTC-3 nuclear extract.	bind
40371	1	9231	5	13	NULL	NULL	NULL	Stn	GP		bind			1-13		Ten1	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0760-0779_embo-j_20_5_11230140_s_5	11230140	A binding defect between Stn1-13 and Ten1 was  responsible for the long telomere phenotype of stn1-13 mutant cells.	bind
40372	2	9231	5	13	NULL	NULL	NULL	statement 1	Process	defect in	is responsible for					long telomere phenotype	Chromosome				NULL	stn1-13 mutant cells	NULL	NULL	NULL	NULL	abs-batch0760-0779_embo-j_20_5_11230140_s_5	11230140	A binding defect between Stn1-13 and Ten1 was  responsible for the long telomere phenotype of stn1-13 mutant cells.	bind
32250	1	9231	6	10	NULL	0	NULL	Stn	NULL		bind	NULL		1-13		Ten1	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0760-0779_embo-j_20_5_11230140_s_5	11230140	A binding defect between Stn1-13 and Ten1 was  responsible for the long telomere phenotype of stn1-13 mutant cells.	bind
32251	2	9231	6	10	NULL	0	NULL	statement 1	NULL	defect in	is responsible for	NULL				long telomere phenotype	NULL				NULL	stn1-13 mutant cells	NULL	NULL	NULL	NULL	abs-batch0760-0779_embo-j_20_5_11230140_s_5	11230140	A binding defect between Stn1-13 and Ten1 was  responsible for the long telomere phenotype of stn1-13 mutant cells.	bind
39696	1	9232	5	13	NULL	NULL	NULL	MANT-ATP	GP		bind					DnaA	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_18_12526_s_122	16517983	A binding experiment fitted with a corresponding saturation function ( Fig. 2 A) showed that the fluorescence intensity of MANT-ATP bound to DnaA increases 1.4-fold.	bind
32252	1	9232	6	NULL	NULL	0	NULL	MANT-ATP	NULL		bind	NULL				DnaA	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_18_12526_s_122	16517983	A binding experiment fitted with a corresponding saturation function ( Fig. 2 A) showed that the fluorescence intensity of MANT-ATP bound to DnaA increases 1.4-fold.	bind
39697	1	9233	5	13	NULL	NULL	NULL	camptothecin	Chemical		bind					DNA-topoisomerase I complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_clinmicrobiolrev_12_4_583_s_40	10515904	A binding model of  the three-dimensional structure of camptothecin (shown in green and labelled CPT)  bound to the DNA-topoisomerase I complex is shown.	bind
32253	1	9233	6	NULL	NULL	0	NULL	camptothecin	NULL		bind	NULL				DNA-topoisomerase I complex	NULL				NULL		0	NULL	NULL	NULL	gw70_clinmicrobiolrev_12_4_583_s_40	10515904	A binding model of  the three-dimensional structure of camptothecin (shown in green and labelled CPT)  bound to the DNA-topoisomerase I complex is shown.	bind
39698	1	9235	5	13	NULL	NULL	NULL	ceramide	Chemical		bind								cysteine-rich C1 domain		NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1634_1_30_s_197	14563411	A binding of ceramide  to a cysteine-rich C1 domain was also suggested for c-Raf [ 8,  10 and   31].	bind
32254	1	9235	6	10	NULL	0	NULL	ceramide	NULL		bind	NULL					NULL		cysteine-rich C1 domain		NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1634_1_30_s_197	14563411	A binding of ceramide  to a cysteine-rich C1 domain was also suggested for c-Raf [ 8,  10 and   31].	bind
39699	1	9236	5	13	NULL	NULL	NULL	FHL2	GP		bind					actin molecules	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_27_28641_s_359	15117962	A binding of FHL2 and FHL3 to actin molecules has recently been published ( ), which would suggest that the LIM-only proteins directly link the cytoskeleton to the ECM via binding to integrins and actin.	bind
39700	2	9236	5	13	NULL	NULL	NULL	FHL3	GP		bind					actin molecules	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_27_28641_s_359	15117962	A binding of FHL2 and FHL3 to actin molecules has recently been published ( ), which would suggest that the LIM-only proteins directly link the cytoskeleton to the ECM via binding to integrins and actin.	bind
39701	3	9236	5	13	NULL	NULL	NULL	cytoskeleton	CellComponent		is linked to		directly			ECM	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_27_28641_s_359	15117962	A binding of FHL2 and FHL3 to actin molecules has recently been published ( ), which would suggest that the LIM-only proteins directly link the cytoskeleton to the ECM via binding to integrins and actin.	bind
39702	4	9236	5	13	NULL	NULL	NULL	LIM-only proteins	GP		is required for					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_27_28641_s_359	15117962	A binding of FHL2 and FHL3 to actin molecules has recently been published ( ), which would suggest that the LIM-only proteins directly link the cytoskeleton to the ECM via binding to integrins and actin.	bind
39703	5	9236	5	13	NULL	NULL	NULL	LIM-only proteins	GP		bind					integrins	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_27_28641_s_359	15117962	A binding of FHL2 and FHL3 to actin molecules has recently been published ( ), which would suggest that the LIM-only proteins directly link the cytoskeleton to the ECM via binding to integrins and actin.	bind
39704	6	9236	5	13	NULL	NULL	NULL	LIM-only proteins	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_27_28641_s_359	15117962	A binding of FHL2 and FHL3 to actin molecules has recently been published ( ), which would suggest that the LIM-only proteins directly link the cytoskeleton to the ECM via binding to integrins and actin.	bind
39705	7	9236	5	13	NULL	NULL	NULL	statement 4	Process		via					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_27_28641_s_359	15117962	A binding of FHL2 and FHL3 to actin molecules has recently been published ( ), which would suggest that the LIM-only proteins directly link the cytoskeleton to the ECM via binding to integrins and actin.	bind
39706	8	9236	5	13	NULL	NULL	NULL	statement 4	Process		via					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_27_28641_s_359	15117962	A binding of FHL2 and FHL3 to actin molecules has recently been published ( ), which would suggest that the LIM-only proteins directly link the cytoskeleton to the ECM via binding to integrins and actin.	bind
49545	9	9236	5	13	NULL	NULL	NULL	FHL2	GP		is a type of					LIM-only proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_27_28641_s_359	15117962	A binding of FHL2 and FHL3 to actin molecules has recently been published ( ), which would suggest that the LIM-only proteins directly link the cytoskeleton to the ECM via binding to integrins and actin.	bind
49546	10	9236	5	13	NULL	NULL	NULL	FHL3	GP		is a type of					LIM-only proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_27_28641_s_359	15117962	A binding of FHL2 and FHL3 to actin molecules has recently been published ( ), which would suggest that the LIM-only proteins directly link the cytoskeleton to the ECM via binding to integrins and actin.	bind
32257	1	9236	6	NULL	NULL	0	NULL	FHL2	NULL		bind	NULL				actin molecules	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_27_28641_s_359	15117962	A binding of FHL2 and FHL3 to actin molecules has recently been published ( ), which would suggest that the LIM-only proteins directly link the cytoskeleton to the ECM via binding to integrins and actin.	bind
32258	2	9236	6	NULL	NULL	0	NULL	FHL3	NULL		bind	NULL				actin molecules	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_27_28641_s_359	15117962	A binding of FHL2 and FHL3 to actin molecules has recently been published ( ), which would suggest that the LIM-only proteins directly link the cytoskeleton to the ECM via binding to integrins and actin.	bind
32259	3	9236	6	NULL	NULL	0	NULL	FHL2	NULL		is a type of	NULL				LIM-only protein	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_27_28641_s_359	15117962	A binding of FHL2 and FHL3 to actin molecules has recently been published ( ), which would suggest that the LIM-only proteins directly link the cytoskeleton to the ECM via binding to integrins and actin.	bind
32260	4	9236	6	NULL	NULL	0	NULL	FHL3	NULL		is a type of	NULL				LIM-only protein	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_27_28641_s_359	15117962	A binding of FHL2 and FHL3 to actin molecules has recently been published ( ), which would suggest that the LIM-only proteins directly link the cytoskeleton to the ECM via binding to integrins and actin.	bind
32261	5	9236	6	NULL	NULL	0	NULL	cytoskeleton	NULL		is linked to	NULL				ECM	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_27_28641_s_359	15117962	A binding of FHL2 and FHL3 to actin molecules has recently been published ( ), which would suggest that the LIM-only proteins directly link the cytoskeleton to the ECM via binding to integrins and actin.	bind
32262	8	9236	6	10	NULL	0	NULL	LIM-only proteins	NULL		is required for	NULL				statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_27_28641_s_359	15117962	A binding of FHL2 and FHL3 to actin molecules has recently been published ( ), which would suggest that the LIM-only proteins directly link the cytoskeleton to the ECM via binding to integrins and actin.	bind
32263	10	9236	6	10	NULL	0	NULL	statement 5	NULL		occurs via	NULL				statement 7	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_27_28641_s_359	15117962	A binding of FHL2 and FHL3 to actin molecules has recently been published ( ), which would suggest that the LIM-only proteins directly link the cytoskeleton to the ECM via binding to integrins and actin.	bind
33275	6	9236	6	10	NULL	0	NULL	LIM-only proteins	NULL		bind	NULL				actin	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_27_28641_s_359	15117962	A binding of FHL2 and FHL3 to actin molecules has recently been published ( ), which would suggest that the LIM-only proteins directly link the cytoskeleton to the ECM via binding to integrins and actin.	bind
33276	9	9236	6	10	NULL	0	NULL	statement 5	NULL		occurs via	NULL				statement 6	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_27_28641_s_359	15117962	A binding of FHL2 and FHL3 to actin molecules has recently been published ( ), which would suggest that the LIM-only proteins directly link the cytoskeleton to the ECM via binding to integrins and actin.	bind
48068	7	9236	6	10	NULL	0	NULL	LIM-only proteins	NULL		bind	NULL				integrins	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_27_28641_s_359	15117962	A binding of FHL2 and FHL3 to actin molecules has recently been published ( ), which would suggest that the LIM-only proteins directly link the cytoskeleton to the ECM via binding to integrins and actin.	bind
39786	1	9237	5	13	NULL	NULL	NULL	MTK1	GP		interact with			N terminus		MTK1	GP		C terminus		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4544_s_341	12052864	A binding of the GADD45 protein to the GADD45-binding site near the autoinhibitory domain will interfere in the autoinhibitory interaction between the MTK1 N and C termini, leading to MKK6 binding and its activation by phosphorylation (Fig.  10B).	bind
39787	2	9237	5	13	NULL	NULL	NULL	statement 1	Process		is					autoinhibitory interaction	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4544_s_341	12052864	A binding of the GADD45 protein to the GADD45-binding site near the autoinhibitory domain will interfere in the autoinhibitory interaction between the MTK1 N and C termini, leading to MKK6 binding and its activation by phosphorylation (Fig.  10B).	bind
39788	3	9237	5	13	NULL	NULL	NULL	GADD45 protein	GP		bind					MTK1	GP		GADD45-binding site near autoinhibitory domain		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4544_s_341	12052864	A binding of the GADD45 protein to the GADD45-binding site near the autoinhibitory domain will interfere in the autoinhibitory interaction between the MTK1 N and C termini, leading to MKK6 binding and its activation by phosphorylation (Fig.  10B).	bind
39789	4	9237	5	13	NULL	NULL	NULL	statement 3	Process		interfere with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4544_s_341	12052864	A binding of the GADD45 protein to the GADD45-binding site near the autoinhibitory domain will interfere in the autoinhibitory interaction between the MTK1 N and C termini, leading to MKK6 binding and its activation by phosphorylation (Fig.  10B).	bind
39790	5	9237	5	13	NULL	NULL	NULL	statement 4	Process		leads to					MKK6	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4544_s_341	12052864	A binding of the GADD45 protein to the GADD45-binding site near the autoinhibitory domain will interfere in the autoinhibitory interaction between the MTK1 N and C termini, leading to MKK6 binding and its activation by phosphorylation (Fig.  10B).	bind
39791	6	9237	5	13	NULL	NULL	NULL	MKK6	GP		undergoes					phosphorylation	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4544_s_341	12052864	A binding of the GADD45 protein to the GADD45-binding site near the autoinhibitory domain will interfere in the autoinhibitory interaction between the MTK1 N and C termini, leading to MKK6 binding and its activation by phosphorylation (Fig.  10B).	bind
39792	7	9237	5	13	NULL	NULL	NULL	statement 6	Process		leads to					MKK6	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4544_s_341	12052864	A binding of the GADD45 protein to the GADD45-binding site near the autoinhibitory domain will interfere in the autoinhibitory interaction between the MTK1 N and C termini, leading to MKK6 binding and its activation by phosphorylation (Fig.  10B).	bind
39793	8	9237	5	13	NULL	NULL	NULL	statement 5	Process		leads to					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4544_s_341	12052864	A binding of the GADD45 protein to the GADD45-binding site near the autoinhibitory domain will interfere in the autoinhibitory interaction between the MTK1 N and C termini, leading to MKK6 binding and its activation by phosphorylation (Fig.  10B).	bind
32533	1	9237	6	10	NULL	0	NULL	GADD45 protein			bind					MTK1			GADD45-binding site		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4544_s_341	12052864	A binding of the GADD45 protein to the GADD45-binding site near the autoinhibitory domain will interfere in the autoinhibitory interaction between the MTK1 N and C termini, leading to MKK6 binding and its activation by phosphorylation (Fig.  10B).	bind
32534	2	9237	6	NULL	NULL	0	NULL		NULL		is located near the	NULL		GADD45-binding site			NULL		autoinhibitory domain		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_13_4544_s_341	12052864	A binding of the GADD45 protein to the GADD45-binding site near the autoinhibitory domain will interfere in the autoinhibitory interaction between the MTK1 N and C termini, leading to MKK6 binding and its activation by phosphorylation (Fig.  10B).	bind
32535	3	9237	6	10	NULL	0	NULL	MTK1			autoinhibits			N terminus		MTK1			C terminus		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_13_4544_s_341	12052864	A binding of the GADD45 protein to the GADD45-binding site near the autoinhibitory domain will interfere in the autoinhibitory interaction between the MTK1 N and C termini, leading to MKK6 binding and its activation by phosphorylation (Fig.  10B).	bind
32536	4	9237	6	NULL	NULL	0	NULL	statement 1	NULL		interferes with	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_13_4544_s_341	12052864	A binding of the GADD45 protein to the GADD45-binding site near the autoinhibitory domain will interfere in the autoinhibitory interaction between the MTK1 N and C termini, leading to MKK6 binding and its activation by phosphorylation (Fig.  10B).	bind
32537	5	9237	6	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				MKK6	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_13_4544_s_341	12052864	A binding of the GADD45 protein to the GADD45-binding site near the autoinhibitory domain will interfere in the autoinhibitory interaction between the MTK1 N and C termini, leading to MKK6 binding and its activation by phosphorylation (Fig.  10B).	bind
32542	6	9237	6	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				MKK6	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_13_4544_s_341	12052864	A binding of the GADD45 protein to the GADD45-binding site near the autoinhibitory domain will interfere in the autoinhibitory interaction between the MTK1 N and C termini, leading to MKK6 binding and its activation by phosphorylation (Fig.  10B).	bind
32546	7	9237	6	NULL	NULL	0	NULL	MKK6	NULL	activation of	occurs by	NULL				phosphorylation	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_13_4544_s_341	12052864	A binding of the GADD45 protein to the GADD45-binding site near the autoinhibitory domain will interfere in the autoinhibitory interaction between the MTK1 N and C termini, leading to MKK6 binding and its activation by phosphorylation (Fig.  10B).	bind
39794	1	9238	5	13	NULL	NULL	NULL	TRs	GP		bind					target genes	GP	Xenopus laevis		TRE	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_8_3204_s_280	16581794	A binding of TRE by TRs has already been reported for  Xenopus laevis target genes ( ).	bind
32264	1	9238	6	NULL	NULL	0	NULL	TR	NULL		bind	NULL				target gene	NULL	Xenopus laevis		TRE	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_8_3204_s_280	16581794	A binding of TRE by TRs has already been reported for  Xenopus laevis target genes ( ).	bind
39795	1	9240	5	13	NULL	NULL	NULL	Pl	GP		bind					fibrin	GP	partially degraded			NULL	purified system with fibrin clots	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27912_s_47	8910391	A binding study in solution and experiments performed in a purified system with fibrin clots demonstrated that STA binds to Pl and to Pg, which is bound to partially degraded fibrin, but does not bind appreciably to Glu-Pg in solution.	bind
39796	2	9240	5	13	NULL	NULL	NULL	STA	GP		bind					statement 1	GP				NULL	purified system with fibrin clots	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27912_s_47	8910391	A binding study in solution and experiments performed in a purified system with fibrin clots demonstrated that STA binds to Pl and to Pg, which is bound to partially degraded fibrin, but does not bind appreciably to Glu-Pg in solution.	bind
39797	3	9240	5	13	NULL	NULL	NULL	Pg	GP		bind					fibrin	GP	partially degraded			NULL	purified system with fibrin clots	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27912_s_47	8910391	A binding study in solution and experiments performed in a purified system with fibrin clots demonstrated that STA binds to Pl and to Pg, which is bound to partially degraded fibrin, but does not bind appreciably to Glu-Pg in solution.	bind
39798	4	9240	5	13	NULL	NULL	NULL	STA	GP		bind					statement 3	GP				NULL	purified system with fibrin clots	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27912_s_47	8910391	A binding study in solution and experiments performed in a purified system with fibrin clots demonstrated that STA binds to Pl and to Pg, which is bound to partially degraded fibrin, but does not bind appreciably to Glu-Pg in solution.	bind
39799	5	9240	5	13	NULL	NULL	NULL	STA	GP		does not bind		appreciably			Glu-Pg	GP				NULL	solution	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27912_s_47	8910391	A binding study in solution and experiments performed in a purified system with fibrin clots demonstrated that STA binds to Pl and to Pg, which is bound to partially degraded fibrin, but does not bind appreciably to Glu-Pg in solution.	bind
32265	1	9240	6	10	NULL	0	NULL	P1			bind					fibrin		partially degraded			NULL	purified system with fibrin clots	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27912_s_47	8910391	A binding study in solution and experiments performed in a purified system with fibrin clots demonstrated that STA binds to Pl and to Pg, which is bound to partially degraded fibrin, but does not bind appreciably to Glu-Pg in solution.	bind
32528	2	9240	6	10	NULL	0	NULL	Pg			bind					fibrin		partially degraded			NULL	purified system with fibrin clots	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27912_s_47	8910391	A binding study in solution and experiments performed in a purified system with fibrin clots demonstrated that STA binds to Pl and to Pg, which is bound to partially degraded fibrin, but does not bind appreciably to Glu-Pg in solution.	bind
32529	3	9240	6	10	NULL	0	NULL	STA			bind					statement 2					NULL	purified system with fibrin clots	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27912_s_47	8910391	A binding study in solution and experiments performed in a purified system with fibrin clots demonstrated that STA binds to Pl and to Pg, which is bound to partially degraded fibrin, but does not bind appreciably to Glu-Pg in solution.	bind
32530	4	9240	6	NULL	NULL	0	NULL	STA	NULL		does not bind	NULL	appreciably			Glu-Pg	NULL				NULL	in solution	0	NULL	NULL	NULL	gw60_jbiolchem_271_44_27912_s_47	8910391	A binding study in solution and experiments performed in a purified system with fibrin clots demonstrated that STA binds to Pl and to Pg, which is bound to partially degraded fibrin, but does not bind appreciably to Glu-Pg in solution.	bind
48069	5	9240	6	10	NULL	0	NULL	STA			bind					statement 1					NULL	purified system with fibrin clots	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27912_s_47	8910391	A binding study in solution and experiments performed in a purified system with fibrin clots demonstrated that STA binds to Pl and to Pg, which is bound to partially degraded fibrin, but does not bind appreciably to Glu-Pg in solution.	bind
39800	1	9241	5	13	NULL	NULL	NULL	RyR3	GP		bind					FKBP12	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_24_17297_s_449	10358090	A binding study with GST-FKBP12 fusion protein revealed that RyR3 can bind FKBP12, as is true of RyR1 (Fig.  3).	bind
39801	2	9241	5	13	NULL	NULL	NULL	RyR1	GP		bind					FKBP12	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_24_17297_s_449	10358090	A binding study with GST-FKBP12 fusion protein revealed that RyR3 can bind FKBP12, as is true of RyR1 (Fig.  3).	bind
32266	1	9241	6	NULL	NULL	0	NULL	RyR3	NULL		bind	NULL				FKBP12	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_24_17297_s_449	10358090	A binding study with GST-FKBP12 fusion protein revealed that RyR3 can bind FKBP12, as is true of RyR1 (Fig.  3).	bind
32267	2	9241	6	NULL	NULL	0	NULL	RyR1	NULL		bind	NULL				FKBP12	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_24_17297_s_449	10358090	A binding study with GST-FKBP12 fusion protein revealed that RyR3 can bind FKBP12, as is true of RyR1 (Fig.  3).	bind
39802	1	9242	5	13	NULL	NULL	NULL	Ca2+	Chemical		bind					CnB	GP				NULL		NULL	NULL	NULL	NULL	gw70_febslett_573_1_121_s_9	15327986	A biochemical approach suggested that the Ca2+-binding to CnB caused to release the CaM-binding domain of CnA from its catalytic  domain to open the active site partially [  11 and   12].	bind
39803	2	9242	5	13	NULL	NULL	NULL	CnA	GP		released from			CaM-binding domain		CnA	GP		catalytic domain		NULL		NULL	NULL	NULL	NULL	gw70_febslett_573_1_121_s_9	15327986	A biochemical approach suggested that the Ca2+-binding to CnB caused to release the CaM-binding domain of CnA from its catalytic  domain to open the active site partially [  11 and   12].	bind
39804	3	9242	5	13	NULL	NULL	NULL	statement 2	Process		open		partially			CnA	GP		active site		NULL		NULL	NULL	NULL	NULL	gw70_febslett_573_1_121_s_9	15327986	A biochemical approach suggested that the Ca2+-binding to CnB caused to release the CaM-binding domain of CnA from its catalytic  domain to open the active site partially [  11 and   12].	bind
39805	4	9242	5	13	NULL	NULL	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_febslett_573_1_121_s_9	15327986	A biochemical approach suggested that the Ca2+-binding to CnB caused to release the CaM-binding domain of CnA from its catalytic  domain to open the active site partially [  11 and   12].	bind
32268	1	9242	6	NULL	NULL	0	NULL	Ca2+	NULL		bind	NULL				CnB	NULL				NULL		0	NULL	NULL	NULL	gw70_febslett_573_1_121_s_9	15327986	A biochemical approach suggested that the Ca2+-binding to CnB caused to release the CaM-binding domain of CnA from its catalytic  domain to open the active site partially [  11 and   12].	bind
32269	2	9242	6	10	NULL	0	NULL	CnA	NULL		release from 	NULL		CaM-binding domain		CnA	NULL		catalytic domain		NULL		NULL	NULL	NULL	NULL	gw70_febslett_573_1_121_s_9	15327986	A biochemical approach suggested that the Ca2+-binding to CnB caused to release the CaM-binding domain of CnA from its catalytic  domain to open the active site partially [  11 and   12].	bind
32324	3	9242	6	NULL	NULL	0	NULL	statement 2	NULL		opens	NULL	partially			active site	NULL				NULL		0	NULL	NULL	NULL	gw70_febslett_573_1_121_s_9	15327986	A biochemical approach suggested that the Ca2+-binding to CnB caused to release the CaM-binding domain of CnA from its catalytic  domain to open the active site partially [  11 and   12].	bind
48070	4	9242	6	10	NULL	0	NULL	statement 1	NULL		leads to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_febslett_573_1_121_s_9	15327986	A biochemical approach suggested that the Ca2+-binding to CnB caused to release the CaM-binding domain of CnA from its catalytic  domain to open the active site partially [  11 and   12].	bind
39806	1	9243	5	13	NULL	NULL	NULL	osteopontin	GP		bind					alpha v beta 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2734_s_367	10733576	A biochemical characterization of the binding of osteopontin to integrins alpha v beta 1 and alpha v beta 5.	bind
39807	2	9243	5	13	NULL	NULL	NULL	alpha v beta 1	GP		is a type of					integrins	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2734_s_367	10733576	A biochemical characterization of the binding of osteopontin to integrins alpha v beta 1 and alpha v beta 5.	bind
39808	3	9243	5	13	NULL	NULL	NULL	osteopontin	GP		bind					alpha v beta 5	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2734_s_367	10733576	A biochemical characterization of the binding of osteopontin to integrins alpha v beta 1 and alpha v beta 5.	bind
39809	4	9243	5	13	NULL	NULL	NULL	alpha v beta 5	GP		is a type of					integrins	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_8_2734_s_367	10733576	A biochemical characterization of the binding of osteopontin to integrins alpha v beta 1 and alpha v beta 5.	bind
32325	1	9243	6	NULL	NULL	0	NULL	osteopontin	NULL		bind	NULL				alpha v beta 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_8_2734_s_367	10733576	A biochemical characterization of the binding of osteopontin to integrins alpha v beta 1 and alpha v beta 5.	bind
32326	2	9243	6	NULL	NULL	0	NULL	osteopontin	NULL		bind	NULL				alpha v beta 5	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_8_2734_s_367	10733576	A biochemical characterization of the binding of osteopontin to integrins alpha v beta 1 and alpha v beta 5.	bind
32327	3	9243	6	NULL	NULL	0	NULL	alpha v beta 5	NULL		is a type of	NULL				integrin	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_8_2734_s_367	10733576	A biochemical characterization of the binding of osteopontin to integrins alpha v beta 1 and alpha v beta 5.	bind
32328	4	9243	6	NULL	NULL	0	NULL	alpha v beta 1	NULL		is a type of	NULL				integrin	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_8_2734_s_367	10733576	A biochemical characterization of the binding of osteopontin to integrins alpha v beta 1 and alpha v beta 5.	bind
39810	1	9245	5	13	NULL	NULL	NULL	ApoE	GP		bind					Abeta	GP	synthetic			NULL	CSF	NULL	NULL	NULL	NULL	gw70_annurevgenomicshum_3_0_67_s_327	null	A biochemical screen for proteins in CSF that bound synthetic Abeta led to  the identification of ApoE as such a protein and to the subsequent recognition that  its gene was in a region of chromosome 19q previously linked to AD in some late-onset  families ( 120).	bind
39811	2	9245	5	13	NULL	NULL	NULL	ApoE gene	GP		is located on					chromosome 19q	Chromosome				NULL		NULL	NULL	NULL	NULL	gw70_annurevgenomicshum_3_0_67_s_327	null	A biochemical screen for proteins in CSF that bound synthetic Abeta led to  the identification of ApoE as such a protein and to the subsequent recognition that  its gene was in a region of chromosome 19q previously linked to AD in some late-onset  families ( 120).	bind
39812	3	9245	5	13	NULL	NULL	NULL	chromosome 19q	Chromosome		is linked to					AD	MedicalFinding				NULL	late-onset families	NULL	NULL	NULL	NULL	gw70_annurevgenomicshum_3_0_67_s_327	null	A biochemical screen for proteins in CSF that bound synthetic Abeta led to  the identification of ApoE as such a protein and to the subsequent recognition that  its gene was in a region of chromosome 19q previously linked to AD in some late-onset  families ( 120).	bind
32524	1	9245	6	10	NULL	0	NULL	ApoE			bind					Abeta		synthetic			NULL	CSF	NULL	NULL	NULL	NULL	gw70_annurevgenomicshum_3_0_67_s_327	null	A biochemical screen for proteins in CSF that bound synthetic Abeta led to  the identification of ApoE as such a protein and to the subsequent recognition that  its gene was in a region of chromosome 19q previously linked to AD in some late-onset  families ( 120).	bind
32525	2	9245	6	10	NULL	0	NULL	ApoE gene			is located on					chromosome 19q					NULL		NULL	NULL	NULL	NULL	gw70_annurevgenomicshum_3_0_67_s_327	null	A biochemical screen for proteins in CSF that bound synthetic Abeta led to  the identification of ApoE as such a protein and to the subsequent recognition that  its gene was in a region of chromosome 19q previously linked to AD in some late-onset  families ( 120).	bind
32527	3	9245	6	10	NULL	0	NULL	statement 2			is linked to					AD 					NULL	late onset families	NULL	NULL	NULL	NULL	gw70_annurevgenomicshum_3_0_67_s_327	null	A biochemical screen for proteins in CSF that bound synthetic Abeta led to  the identification of ApoE as such a protein and to the subsequent recognition that  its gene was in a region of chromosome 19q previously linked to AD in some late-onset  families ( 120).	bind
39813	2	9246	5	13	NULL	NULL	NULL	statement 1	GP		bind					HLA-E	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_23_0_225_s_299	15771571	A biological consequence of this is suggested by the studies of Michaelsson and  colleagues ( 212), who have shown that peptides derived from heat shock protein 60 (hsp60) bind to  HLA-E; however, these HLA-E molecules containing hsp60 peptides are not able to bind  the inhibitory CD94/NKG2A receptor.	bind
39814	3	9246	5	13	NULL	NULL	NULL	statement 2	GP		does not bind					CD94/NKG2A	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_23_0_225_s_299	15771571	A biological consequence of this is suggested by the studies of Michaelsson and  colleagues ( 212), who have shown that peptides derived from heat shock protein 60 (hsp60) bind to  HLA-E; however, these HLA-E molecules containing hsp60 peptides are not able to bind  the inhibitory CD94/NKG2A receptor.	bind
48071	1	9246	5	13	NULL	NULL	NULL	peptide	GP		derived from					hsp60	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_23_0_225_s_299	15771571	A biological consequence of this is suggested by the studies of Michaelsson and  colleagues ( 212), who have shown that peptides derived from heat shock protein 60 (hsp60) bind to  HLA-E; however, these HLA-E molecules containing hsp60 peptides are not able to bind  the inhibitory CD94/NKG2A receptor.	bind
48072	4	9246	5	13	NULL	NULL	NULL	CD94/NKG2A	GP		is a type of					inhibitory receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_23_0_225_s_299	15771571	A biological consequence of this is suggested by the studies of Michaelsson and  colleagues ( 212), who have shown that peptides derived from heat shock protein 60 (hsp60) bind to  HLA-E; however, these HLA-E molecules containing hsp60 peptides are not able to bind  the inhibitory CD94/NKG2A receptor.	bind
48073	5	9246	5	13	NULL	NULL	NULL	hsp60	GP		is					heat shock protein 60	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_23_0_225_s_299	15771571	A biological consequence of this is suggested by the studies of Michaelsson and  colleagues ( 212), who have shown that peptides derived from heat shock protein 60 (hsp60) bind to  HLA-E; however, these HLA-E molecules containing hsp60 peptides are not able to bind  the inhibitory CD94/NKG2A receptor.	bind
32329	1	9246	6	10	NULL	0	NULL	peptides	NULL		derived from	NULL				hsp60	NULL				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_23_0_225_s_299	15771571	A biological consequence of this is suggested by the studies of Michaelsson and  colleagues ( 212), who have shown that peptides derived from heat shock protein 60 (hsp60) bind to  HLA-E; however, these HLA-E molecules containing hsp60 peptides are not able to bind  the inhibitory CD94/NKG2A receptor.	bind
32330	2	9246	6	10	NULL	0	NULL	statement 1	NULL		bind	NULL				HLA-E	NULL				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_23_0_225_s_299	15771571	A biological consequence of this is suggested by the studies of Michaelsson and  colleagues ( 212), who have shown that peptides derived from heat shock protein 60 (hsp60) bind to  HLA-E; however, these HLA-E molecules containing hsp60 peptides are not able to bind  the inhibitory CD94/NKG2A receptor.	bind
32331	3	9246	6	NULL	NULL	0	NULL	statement 2	NULL		does not bind	NULL				CD94/NKG2A 	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_23_0_225_s_299	15771571	A biological consequence of this is suggested by the studies of Michaelsson and  colleagues ( 212), who have shown that peptides derived from heat shock protein 60 (hsp60) bind to  HLA-E; however, these HLA-E molecules containing hsp60 peptides are not able to bind  the inhibitory CD94/NKG2A receptor.	bind
32332	4	9246	6	NULL	NULL	0	NULL	CD94/NKG2A	NULL		is a type of	NULL				inhibitory receptor	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_23_0_225_s_299	15771571	A biological consequence of this is suggested by the studies of Michaelsson and  colleagues ( 212), who have shown that peptides derived from heat shock protein 60 (hsp60) bind to  HLA-E; however, these HLA-E molecules containing hsp60 peptides are not able to bind  the inhibitory CD94/NKG2A receptor.	bind
48074	5	9246	6	10	NULL	0	NULL	hsp60	NULL		is	NULL				heat shock protein 60	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_23_0_225_s_299	15771571	A biological consequence of this is suggested by the studies of Michaelsson and  colleagues ( 212), who have shown that peptides derived from heat shock protein 60 (hsp60) bind to  HLA-E; however, these HLA-E molecules containing hsp60 peptides are not able to bind  the inhibitory CD94/NKG2A receptor.	bind
39815	1	9247	5	13	NULL	NULL	NULL	p85alpha	GP		bind			SH2 domains		Tyr(P) peptide	AminoAcid	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_22_15678_s_143	10336465	A biosensor-based competition assay was used to measure the binding of p85alpha SH2 domains to an immobilized Tyr(P) peptide with the sequence DMSKDESVDY(P)VPMLDMK (Y(P) is phosphotyrosine).	bind
39816	2	9247	5	13	NULL	NULL	NULL	Y(P)	AminoAcid		is					phosphotyrosine	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_22_15678_s_143	10336465	A biosensor-based competition assay was used to measure the binding of p85alpha SH2 domains to an immobilized Tyr(P) peptide with the sequence DMSKDESVDY(P)VPMLDMK (Y(P) is phosphotyrosine).	bind
48075	3	9247	5	13	NULL	NULL	NULL	Tyr(P) peptide	AminoAcid		is					DMSKDESVDY(P)VPMLDMK	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_22_15678_s_143	10336465	A biosensor-based competition assay was used to measure the binding of p85alpha SH2 domains to an immobilized Tyr(P) peptide with the sequence DMSKDESVDY(P)VPMLDMK (Y(P) is phosphotyrosine).	bind
32333	1	9247	6	NULL	NULL	0	NULL	p85alpha	NULL		bind	NULL		SH2 domain		Tyr(P) peptide	NULL	immobilized			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_22_15678_s_143	10336465	A biosensor-based competition assay was used to measure the binding of p85alpha SH2 domains to an immobilized Tyr(P) peptide with the sequence DMSKDESVDY(P)VPMLDMK (Y(P) is phosphotyrosine).	bind
32334	2	9247	6	NULL	NULL	0	NULL	Tyr(P) peptide	NULL		is	NULL				DMSKDESVDY(P)VPMLDMK	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_22_15678_s_143	10336465	A biosensor-based competition assay was used to measure the binding of p85alpha SH2 domains to an immobilized Tyr(P) peptide with the sequence DMSKDESVDY(P)VPMLDMK (Y(P) is phosphotyrosine).	bind
32335	3	9247	6	NULL	NULL	0	NULL	Y(P)	NULL		is	NULL				phosphotyrosine	NULL				NULL	statement 2	0	NULL	NULL	NULL	gw60_jbiolchem_274_22_15678_s_143	10336465	A biosensor-based competition assay was used to measure the binding of p85alpha SH2 domains to an immobilized Tyr(P) peptide with the sequence DMSKDESVDY(P)VPMLDMK (Y(P) is phosphotyrosine).	bind
39817	1	9248	5	13	NULL	NULL	NULL	ParB	GP		bind					 DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_2_427_s_117	12191487	A biotinylated 26 bp double-stranded oligonucleotide containing sequence of the ParB binding site within the  gidABparAB operon promoter region was immobilized on a streptavidin sensor chip and used to investigate the effects of ParA on ParB DNA binding activity by SPR.	bind
32336	1	9248	6	NULL	NULL	0	NULL	ParB	NULL		bind	NULL				DNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcell_10_2_427_s_117	12191487	A biotinylated 26 bp double-stranded oligonucleotide containing sequence of the ParB binding site within the  gidABparAB operon promoter region was immobilized on a streptavidin sensor chip and used to investigate the effects of ParA on ParB DNA binding activity by SPR.	bind
39818	1	9250	5	13	NULL	NULL	NULL	ATr	GP	biotinylated;;mutant	does not bind					MEF-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7575_s_309	11096067	A biotinylated mutant ATr did not bind to either MEF-2 or p300 (data not shown).	bind
39819	2	9250	5	13	NULL	NULL	NULL	ATr	GP	biotinylated;;mutant	does not bind					p300	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7575_s_309	11096067	A biotinylated mutant ATr did not bind to either MEF-2 or p300 (data not shown).	bind
39820	3	9250	5	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7575_s_309	11096067	A biotinylated mutant ATr did not bind to either MEF-2 or p300 (data not shown).	bind
32339	1	9250	6	NULL	NULL	0	NULL	ATr	NULL	biotinylated;; mutant	does not bind	NULL				MEF-2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_10_7575_s_309	11096067	A biotinylated mutant ATr did not bind to either MEF-2 or p300 (data not shown).	bind
32340	2	9250	6	NULL	NULL	0	NULL	ATr	NULL	biotinylated;; mutant	does not bind	NULL				p300	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_10_7575_s_309	11096067	A biotinylated mutant ATr did not bind to either MEF-2 or p300 (data not shown).	bind
48076	3	9250	6	10	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_10_7575_s_309	11096067	A biotinylated mutant ATr did not bind to either MEF-2 or p300 (data not shown).	bind
39821	1	9251	5	13	NULL	NULL	NULL	21 aa peptide	GP	biotinylated;;Plasmodium falciparum	bind					glycophorin A	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_9_4203_s_2	9712768	A biotinylated peptide covering a sequence of 21 amino acids (aa) from the erythrocyte binding antigen (EBA-175) of  Plasmodium falciparum bound to human glycophorin A, an erythrocyte receptor for merozoites, as demonstrated by enzyme-linked immunosorbent assay (ELISA) and to erythrocytes as demonstrated by flow cytometry analysis.	bind
39822	2	9251	5	13	NULL	NULL	NULL	glycophorin A	GP		is a type of					erythrocyte receptor for merozoites	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_9_4203_s_2	9712768	A biotinylated peptide covering a sequence of 21 amino acids (aa) from the erythrocyte binding antigen (EBA-175) of  Plasmodium falciparum bound to human glycophorin A, an erythrocyte receptor for merozoites, as demonstrated by enzyme-linked immunosorbent assay (ELISA) and to erythrocytes as demonstrated by flow cytometry analysis.	bind
39823	3	9251	5	13	NULL	NULL	NULL	21 aa peptide 	GP	biotinylated;;Plasmodium falciparum	bind					erythrocytes	Cell				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_9_4203_s_2	9712768	A biotinylated peptide covering a sequence of 21 amino acids (aa) from the erythrocyte binding antigen (EBA-175) of  Plasmodium falciparum bound to human glycophorin A, an erythrocyte receptor for merozoites, as demonstrated by enzyme-linked immunosorbent assay (ELISA) and to erythrocytes as demonstrated by flow cytometry analysis.	bind
48077	4	9251	5	13	NULL	NULL	NULL	21 aa peptide	GP		is derived from					EBA-175	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_9_4203_s_2	9712768	A biotinylated peptide covering a sequence of 21 amino acids (aa) from the erythrocyte binding antigen (EBA-175) of  Plasmodium falciparum bound to human glycophorin A, an erythrocyte receptor for merozoites, as demonstrated by enzyme-linked immunosorbent assay (ELISA) and to erythrocytes as demonstrated by flow cytometry analysis.	bind
48078	5	9251	5	13	NULL	NULL	NULL	EBA	GP		is					erythrocyte binding antigen	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_9_4203_s_2	9712768	A biotinylated peptide covering a sequence of 21 amino acids (aa) from the erythrocyte binding antigen (EBA-175) of  Plasmodium falciparum bound to human glycophorin A, an erythrocyte receptor for merozoites, as demonstrated by enzyme-linked immunosorbent assay (ELISA) and to erythrocytes as demonstrated by flow cytometry analysis.	bind
32456	1	9251	6	NULL	NULL	0	NULL	EBA	NULL		is	NULL				erythrocyte binding antigen	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_9_4203_s_2	9712768	A biotinylated peptide covering a sequence of 21 amino acids (aa) from the erythrocyte binding antigen (EBA-175) of  Plasmodium falciparum bound to human glycophorin A, an erythrocyte receptor for merozoites, as demonstrated by enzyme-linked immunosorbent assay (ELISA) and to erythrocytes as demonstrated by flow cytometry analysis.	bind
32457	2	9251	6	10	NULL	0	NULL	 21 aa peptide 	NULL	biotinylated;; Plasmodium falciparum	bind	NULL				glycophorin A	NULL	human			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_9_4203_s_2	9712768	A biotinylated peptide covering a sequence of 21 amino acids (aa) from the erythrocyte binding antigen (EBA-175) of  Plasmodium falciparum bound to human glycophorin A, an erythrocyte receptor for merozoites, as demonstrated by enzyme-linked immunosorbent assay (ELISA) and to erythrocytes as demonstrated by flow cytometry analysis.	bind
32458	3	9251	6	NULL	NULL	0	NULL	glycophorin A	NULL		is a type of	NULL				erythrocyte receptor for merozoites	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_9_4203_s_2	9712768	A biotinylated peptide covering a sequence of 21 amino acids (aa) from the erythrocyte binding antigen (EBA-175) of  Plasmodium falciparum bound to human glycophorin A, an erythrocyte receptor for merozoites, as demonstrated by enzyme-linked immunosorbent assay (ELISA) and to erythrocytes as demonstrated by flow cytometry analysis.	bind
48079	4	9251	6	10	NULL	0	NULL	21 aa peptide	NULL		bind	NULL				erythrocytes	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_9_4203_s_2	9712768	A biotinylated peptide covering a sequence of 21 amino acids (aa) from the erythrocyte binding antigen (EBA-175) of  Plasmodium falciparum bound to human glycophorin A, an erythrocyte receptor for merozoites, as demonstrated by enzyme-linked immunosorbent assay (ELISA) and to erythrocytes as demonstrated by flow cytometry analysis.	bind
48080	5	9251	6	10	NULL	0	NULL	21 aa peptide	NULL		is derived from	NULL				EBA-175	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_9_4203_s_2	9712768	A biotinylated peptide covering a sequence of 21 amino acids (aa) from the erythrocyte binding antigen (EBA-175) of  Plasmodium falciparum bound to human glycophorin A, an erythrocyte receptor for merozoites, as demonstrated by enzyme-linked immunosorbent assay (ELISA) and to erythrocytes as demonstrated by flow cytometry analysis.	bind
39824	1	9254	5	13	NULL	NULL	NULL	citron protein	GP	mouse	bind					GTP-Rho	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_19_1_96_s_123	9870942	A BLAST search of the GenBank database revealed that the remaining four peptide sequences (Table  1) are present in a protein named citron previously identified in mouse by the yeast two-hybrid method as a GTP-Rho binding partner and proposed to be a Rho/ac effector (Madaule et al., 1995  ).	bind
39825	2	9254	5	13	NULL	NULL	NULL	citron protein	GP		is a type of					Rho/ac effector	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_19_1_96_s_123	9870942	A BLAST search of the GenBank database revealed that the remaining four peptide sequences (Table  1) are present in a protein named citron previously identified in mouse by the yeast two-hybrid method as a GTP-Rho binding partner and proposed to be a Rho/ac effector (Madaule et al., 1995  ).	bind
32343	1	9254	6	10	NULL	0	NULL	citron	NULL		is a type of	NULL				Rho/ac effector	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_19_1_96_s_123	9870942	A BLAST search of the GenBank database revealed that the remaining four peptide sequences (Table  1) are present in a protein named citron previously identified in mouse by the yeast two-hybrid method as a GTP-Rho binding partner and proposed to be a Rho/ac effector (Madaule et al., 1995  ).	bind
32344	2	9254	6	NULL	NULL	0	NULL	citron	NULL	mouse	bind	NULL				GTP-Rho	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_1_96_s_123	9870942	A BLAST search of the GenBank database revealed that the remaining four peptide sequences (Table  1) are present in a protein named citron previously identified in mouse by the yeast two-hybrid method as a GTP-Rho binding partner and proposed to be a Rho/ac effector (Madaule et al., 1995  ).	bind
39827	1	9256	5	13	NULL	NULL	NULL	Mpeg1	GP	mouse	expressed in		predominantly			macrophage	Cell	mammalian			NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_468_s_7	15020241	A BLAST search [  17] of the sequences identified a homolog of mouse and human macrophage expressed gene  1 (Mpeg1), a protein thought at that time to be expressed predominantly in mammalian  macrophage [  18].	bind
39828	2	9256	5	13	NULL	NULL	NULL	Mpeg1	GP	human	expressed in		predominantly			macrophage	Cell	mammalian			NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_468_s_7	15020241	A BLAST search [  17] of the sequences identified a homolog of mouse and human macrophage expressed gene  1 (Mpeg1), a protein thought at that time to be expressed predominantly in mammalian  macrophage [  18].	bind
39829	3	9256	5	13	NULL	NULL	NULL	Mpeg1	GP		is					macrophage expressed gene 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_468_s_7	15020241	A BLAST search [  17] of the sequences identified a homolog of mouse and human macrophage expressed gene  1 (Mpeg1), a protein thought at that time to be expressed predominantly in mammalian  macrophage [  18].	bind
32345	1	9256	6	NULL	NULL	0	NULL	Mpeg1	NULL		is	NULL				macrophage expressed gene 1	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_468_s_7	15020241	A BLAST search [  17] of the sequences identified a homolog of mouse and human macrophage expressed gene  1 (Mpeg1), a protein thought at that time to be expressed predominantly in mammalian  macrophage [  18].	bind
32346	2	9256	6	10	NULL	0	NULL	Mpeg1		mouse	is expressed in		predominantly			macrophage		mammalian			NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_468_s_7	15020241	A BLAST search [  17] of the sequences identified a homolog of mouse and human macrophage expressed gene  1 (Mpeg1), a protein thought at that time to be expressed predominantly in mammalian  macrophage [  18].	bind
57861	3	9256	6	10	NULL	0	NULL	Mpeg1		human	expressed in		predominantly			macrophage		mammalian			NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_468_s_7	15020241	A BLAST search [  17] of the sequences identified a homolog of mouse and human macrophage expressed gene  1 (Mpeg1), a protein thought at that time to be expressed predominantly in mammalian  macrophage [  18].	bind
39830	1	9257	5	13	NULL	NULL	NULL	MSG1	GP		bind		specifically			p300	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_12_8825_s_99	10722728	A blocking peptide that disrupted binding of p300 to the anti-p300 antibody abolished the coprecipitation of MSG1 with p300 (Fig.  2 A), demonstrating that the MSG1 coprecipitation was specific.	bind
48081	2	9257	5	13	NULL	NULL	NULL	p300	GP		bind					anti-p300 antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_12_8825_s_99	10722728	A blocking peptide that disrupted binding of p300 to the anti-p300 antibody abolished the coprecipitation of MSG1 with p300 (Fig.  2 A), demonstrating that the MSG1 coprecipitation was specific.	bind
48082	3	9257	5	13	NULL	NULL	NULL	blocking peptide	GP		disrupts					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_12_8825_s_99	10722728	A blocking peptide that disrupted binding of p300 to the anti-p300 antibody abolished the coprecipitation of MSG1 with p300 (Fig.  2 A), demonstrating that the MSG1 coprecipitation was specific.	bind
48083	4	9257	5	13	NULL	NULL	NULL	blocking peptide	GP		abolish					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_12_8825_s_99	10722728	A blocking peptide that disrupted binding of p300 to the anti-p300 antibody abolished the coprecipitation of MSG1 with p300 (Fig.  2 A), demonstrating that the MSG1 coprecipitation was specific.	bind
32347	1	9257	6	10	NULL	0	NULL	MSG1	NULL		bind	NULL	specifically			p300	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_12_8825_s_99	10722728	A blocking peptide that disrupted binding of p300 to the anti-p300 antibody abolished the coprecipitation of MSG1 with p300 (Fig.  2 A), demonstrating that the MSG1 coprecipitation was specific.	bind
32363	2	9257	6	NULL	NULL	0	NULL	p300	NULL		bind	NULL				anti-p300 antibody	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_12_8825_s_99	10722728	A blocking peptide that disrupted binding of p300 to the anti-p300 antibody abolished the coprecipitation of MSG1 with p300 (Fig.  2 A), demonstrating that the MSG1 coprecipitation was specific.	bind
32364	3	9257	6	NULL	NULL	0	NULL	blocking peptide	NULL		disrupts	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_12_8825_s_99	10722728	A blocking peptide that disrupted binding of p300 to the anti-p300 antibody abolished the coprecipitation of MSG1 with p300 (Fig.  2 A), demonstrating that the MSG1 coprecipitation was specific.	bind
32365	4	9257	6	NULL	NULL	0	NULL	blocking peptide	NULL		abolishes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_12_8825_s_99	10722728	A blocking peptide that disrupted binding of p300 to the anti-p300 antibody abolished the coprecipitation of MSG1 with p300 (Fig.  2 A), demonstrating that the MSG1 coprecipitation was specific.	bind
39904	1	9258	5	13	NULL	NULL	NULL	dopamine	Chemical		bind		directly			NMDA receptor-channel macromolecule	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_126_8_1847_s_158	10372829	A blocking rate of the order of tens of milliseconds was not to be expected if the effect were mediated by a metabotropic pathway, and in turn suggests that dopamine was binding directly to the NMDA receptor-channel macromolecule.	bind
32421	1	9258	6	NULL	NULL	0	NULL	dopamine	NULL		bind	NULL	directly			NMDA receptor-channel macromolecule	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_126_8_1847_s_158	10372829	A blocking rate of the order of tens of milliseconds was not to be expected if the effect were mediated by a metabotropic pathway, and in turn suggests that dopamine was binding directly to the NMDA receptor-channel macromolecule.	bind
39905	1	9259	5	13	NULL	NULL	NULL	BMPR-II	GP	mutant	contains								COOH-terminal truncation		NULL	PPH	NULL	NULL	NULL	NULL	abs-batch0560-0569_j-cell-biol_162_6_12963706_s_8	12963706	A BMPR-II mutant containing  the smallest COOH-terminal truncation described in PPH failed to bind  or inhibit LIMK1.	bind
39906	2	9259	5	13	NULL	NULL	NULL	statement 1	GP		does not bind					LIMK1	GP				NULL	PPH	NULL	NULL	NULL	NULL	abs-batch0560-0569_j-cell-biol_162_6_12963706_s_8	12963706	A BMPR-II mutant containing  the smallest COOH-terminal truncation described in PPH failed to bind  or inhibit LIMK1.	bind
39907	3	9259	5	13	NULL	NULL	NULL	statement 1	GP		does not inhibit					LIMK1	GP				NULL	PPH	NULL	NULL	NULL	NULL	abs-batch0560-0569_j-cell-biol_162_6_12963706_s_8	12963706	A BMPR-II mutant containing  the smallest COOH-terminal truncation described in PPH failed to bind  or inhibit LIMK1.	bind
32424	1	9259	6	10	NULL	0	NULL	BMPR-II		mutant;; truncated	does not bind			COOH terminus		LIMK1					NULL	PPH	NULL	NULL	NULL	NULL	abs-batch0560-0569_j-cell-biol_162_6_12963706_s_8	12963706	A BMPR-II mutant containing  the smallest COOH-terminal truncation described in PPH failed to bind  or inhibit LIMK1.	bind
32437	2	9259	6	10	NULL	0	NULL	BMPR-II		mutant;; truncated	does not inhibit			COOH terminus		LIMK1					NULL	PPH	NULL	NULL	NULL	NULL	abs-batch0560-0569_j-cell-biol_162_6_12963706_s_8	12963706	A BMPR-II mutant containing  the smallest COOH-terminal truncation described in PPH failed to bind  or inhibit LIMK1.	bind
39908	1	9261	5	13	NULL	NULL	NULL	BmrR dimer	GP		bind					bmr DNA	NucleicAcid			promoter	NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_299	12456787	A BmrR dimer concurrently bound to both  bmr promoter DNA and drugs (D) can correctly orient the -10 and -35 hexamers of this  promoter to facilitate the binding of RNA polymerase.	bind
39909	2	9261	5	13	NULL	NULL	NULL	BmrR dimer	GP		bind					drug	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_299	12456787	A BmrR dimer concurrently bound to both  bmr promoter DNA and drugs (D) can correctly orient the -10 and -35 hexamers of this  promoter to facilitate the binding of RNA polymerase.	bind
39910	3	9261	5	13	NULL	NULL	NULL	statement 1	Process		concurrent to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_299	12456787	A BmrR dimer concurrently bound to both  bmr promoter DNA and drugs (D) can correctly orient the -10 and -35 hexamers of this  promoter to facilitate the binding of RNA polymerase.	bind
39911	4	9261	5	13	NULL	NULL	NULL	BmrR dimer	GP		orient		correctly			bmr DNA	NucleicAcid			-10 and -35 hexamers of promoter	NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_299	12456787	A BmrR dimer concurrently bound to both  bmr promoter DNA and drugs (D) can correctly orient the -10 and -35 hexamers of this  promoter to facilitate the binding of RNA polymerase.	bind
39912	5	9261	5	13	NULL	NULL	NULL	statement 4	Process		facilitates					RNA polymerase	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_299	12456787	A BmrR dimer concurrently bound to both  bmr promoter DNA and drugs (D) can correctly orient the -10 and -35 hexamers of this  promoter to facilitate the binding of RNA polymerase.	bind
57863	6	9261	5	13	NULL	NULL	NULL	D	Chemical		is					drugs	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_299	12456787	A BmrR dimer concurrently bound to both  bmr promoter DNA and drugs (D) can correctly orient the -10 and -35 hexamers of this  promoter to facilitate the binding of RNA polymerase.	bind
32445	1	9261	6	10	NULL	0	NULL	BmrR dimer			bind					bmr DNA				promoter	NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_299	12456787	A BmrR dimer concurrently bound to both  bmr promoter DNA and drugs (D) can correctly orient the -10 and -35 hexamers of this  promoter to facilitate the binding of RNA polymerase.	bind
32446	2	9261	6	10	NULL	0	NULL	BmrR dimer	NULL		orient	NULL				bmr 	NULL			-10 and -35 hexamers of promoter	NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_299	12456787	A BmrR dimer concurrently bound to both  bmr promoter DNA and drugs (D) can correctly orient the -10 and -35 hexamers of this  promoter to facilitate the binding of RNA polymerase.	bind
32453	3	9261	6	10	NULL	0	NULL	BmrR dimer	NULL		bind	NULL				drug	NULL				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_299	12456787	A BmrR dimer concurrently bound to both  bmr promoter DNA and drugs (D) can correctly orient the -10 and -35 hexamers of this  promoter to facilitate the binding of RNA polymerase.	bind
32454	4	9261	6	10	NULL	0	NULL	statement 2	NULL		facilitates	NULL				RNA polymerase	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_299	12456787	A BmrR dimer concurrently bound to both  bmr promoter DNA and drugs (D) can correctly orient the -10 and -35 hexamers of this  promoter to facilitate the binding of RNA polymerase.	bind
32455	5	9261	6	NULL	NULL	0	NULL	D	NULL		is	NULL				drugs	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_299	12456787	A BmrR dimer concurrently bound to both  bmr promoter DNA and drugs (D) can correctly orient the -10 and -35 hexamers of this  promoter to facilitate the binding of RNA polymerase.	bind
57862	6	9261	6	10	NULL	0	NULL	statement 1			concurrent to					statement 3					NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_299	12456787	A BmrR dimer concurrently bound to both  bmr promoter DNA and drugs (D) can correctly orient the -10 and -35 hexamers of this  promoter to facilitate the binding of RNA polymerase.	bind
39913	1	9263	5	13	NULL	NULL	NULL	MD-2	GP		bind					TLR4	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_17_11955_s_258	16467306	A body of evidence points to structural differences of MD-2 bound to TLR4 and soluble MD-2.	bind
48084	2	9263	5	13	NULL	NULL	NULL	MD-2	GP		bind					MD-2	GP	soluble			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_17_11955_s_258	16467306	A body of evidence points to structural differences of MD-2 bound to TLR4 and soluble MD-2.	bind
32447	1	9263	6	NULL	NULL	0	NULL	MD-2	NULL		bind	NULL				TLR4	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_17_11955_s_258	16467306	A body of evidence points to structural differences of MD-2 bound to TLR4 and soluble MD-2.	bind
32448	2	9263	6	NULL	NULL	0	NULL	MD-2	NULL		bind	NULL				MD-2	NULL	soluble			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_17_11955_s_258	16467306	A body of evidence points to structural differences of MD-2 bound to TLR4 and soluble MD-2.	bind
39915	1	9264	5	13	NULL	NULL	NULL	MPD molecule	Chemical	bound	identifies							putative	GlcNAc binding pocket		NULL		NULL	NULL	NULL	NULL	gw60_embo_20_12_3008_s_175	11406577	A bound MPD molecule identifies a putative GlcNAc binding pocket, located near the active site, and enables a hypothesis explaining the enzyme s dependency on the single GlcNAc substitution of the GlcNAcMan5GlcNAc2 substrate for binding.	bind
39916	2	9264	5	10	NULL	0	NULL			putative	is located near			GlcNAc binding pocket					active site		NULL		NULL	NULL	NULL	NULL	gw60_embo_20_12_3008_s_175	11406577	A bound MPD molecule identifies a putative GlcNAc binding pocket, located near the active site, and enables a hypothesis explaining the enzyme s dependency on the single GlcNAc substitution of the GlcNAcMan5GlcNAc2 substrate for binding.	bind
39919	3	9264	5	13	NULL	NULL	NULL	GlcNAc	Chemical	single	is substituted in					GlcNAcMan5GlcNAc2 substrate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_12_3008_s_175	11406577	A bound MPD molecule identifies a putative GlcNAc binding pocket, located near the active site, and enables a hypothesis explaining the enzyme s dependency on the single GlcNAc substitution of the GlcNAcMan5GlcNAc2 substrate for binding.	bind
39920	4	9264	5	13	NULL	NULL	NULL	enzyme	GP	binding of	depends on		potentially			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_12_3008_s_175	11406577	A bound MPD molecule identifies a putative GlcNAc binding pocket, located near the active site, and enables a hypothesis explaining the enzyme s dependency on the single GlcNAc substitution of the GlcNAcMan5GlcNAc2 substrate for binding.	bind
32450	1	9264	6	NULL	NULL	0	NULL	MPD molecule	NULL	bound	identifies	NULL					NULL	putative	GlcNAc binding pocket		NULL		0	NULL	NULL	NULL	gw60_embo_20_12_3008_s_175	11406577	A bound MPD molecule identifies a putative GlcNAc binding pocket, located near the active site, and enables a hypothesis explaining the enzyme s dependency on the single GlcNAc substitution of the GlcNAcMan5GlcNAc2 substrate for binding.	bind
32451	2	9264	6	NULL	NULL	0	NULL	GlcNAcMan5GlcNAc2 substrate	NULL	binding of	is dependent on	NULL				GlcNAc	NULL	substitution of 			NULL		0	NULL	NULL	NULL	gw60_embo_20_12_3008_s_175	11406577	A bound MPD molecule identifies a putative GlcNAc binding pocket, located near the active site, and enables a hypothesis explaining the enzyme s dependency on the single GlcNAc substitution of the GlcNAcMan5GlcNAc2 substrate for binding.	bind
32452	3	9264	6	NULL	NULL	0	NULL	statement 2	NULL		enables	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_20_12_3008_s_175	11406577	A bound MPD molecule identifies a putative GlcNAc binding pocket, located near the active site, and enables a hypothesis explaining the enzyme s dependency on the single GlcNAc substitution of the GlcNAcMan5GlcNAc2 substrate for binding.	bind
57864	4	9264	6	10	NULL	0	NULL			putative	is located near			GlcNAc binding pocket					active site		NULL		NULL	NULL	NULL	NULL	gw60_embo_20_12_3008_s_175	11406577	A bound MPD molecule identifies a putative GlcNAc binding pocket, located near the active site, and enables a hypothesis explaining the enzyme s dependency on the single GlcNAc substitution of the GlcNAcMan5GlcNAc2 substrate for binding.	bind
39921	1	9265	5	13	NULL	NULL	NULL	papillomavirus E1-related protein	GP	bovine	bind		specifically			papillomavirus DNA	NucleicAcid	bovine			NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_1_149_s_527	10949036	A bovine papillomavirus E1-related protein binds specifically to bovine papillomavirus DNA.	bind
32449	1	9265	6	NULL	NULL	0	NULL	papillomavirus E1-related protein	NULL	bovine	bind	NULL	specifically			papillomavirus DNA	NULL	bovine			NULL		0	NULL	NULL	NULL	gw60_molcell_6_1_149_s_527	10949036	A bovine papillomavirus E1-related protein binds specifically to bovine papillomavirus DNA.	bind
39931	1	9267	5	13	NULL	NULL	NULL	Cdc42	GP		activate					serine/threonine protein kinase	GP	brain			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6354_s_491	10938112	A brain serine/threonine protein kinase activated by Cdc42 and Rac1.	bind
39932	2	9267	5	13	NULL	NULL	NULL	Rac1	GP		activates					serine/threonine protein kinase	GP	brain			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6354_s_491	10938112	A brain serine/threonine protein kinase activated by Cdc42 and Rac1.	bind
32570	1	9267	6	10	NULL	0	NULL	serine/threonine protein kinase		brain 	is activated by					Cdc42					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6354_s_491	10938112	A brain serine/threonine protein kinase activated by Cdc42 and Rac1.	bind
32571	2	9267	6	10	NULL	0	NULL	 serine/threonine protein kinase		brain	is activated by					Rac1					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6354_s_491	10938112	A brain serine/threonine protein kinase activated by Cdc42 and Rac1.	bind
39933	1	9268	5	13	NULL	NULL	NULL	chondroitin sulfate proteoglycan	GP	brain-derived	is related to					phosphacan	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_19_11_4245_s_45	10341229	A brain-derived chondroitin sulfate proteoglycan related to phosphacan has been isolated by affinity to a recombinant amino-terminal EGF domain of TN-R (Xiao et al., 1997  ), and phosphacan binds with high affinity ( Kd ~2 nM) to native TN-R (Milev et al., 1998  ).	bind
39934	2	9268	5	13	NULL	NULL	NULL	statement 1	GP		bind					TN-R	GP	recombinant	amino-terminal EGF domain		NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_19_11_4245_s_45	10341229	A brain-derived chondroitin sulfate proteoglycan related to phosphacan has been isolated by affinity to a recombinant amino-terminal EGF domain of TN-R (Xiao et al., 1997  ), and phosphacan binds with high affinity ( Kd ~2 nM) to native TN-R (Milev et al., 1998  ).	bind
39935	3	9268	5	13	NULL	NULL	NULL	phosphacan	GP		bind		high affinity			TN-R	GP	native			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_19_11_4245_s_45	10341229	A brain-derived chondroitin sulfate proteoglycan related to phosphacan has been isolated by affinity to a recombinant amino-terminal EGF domain of TN-R (Xiao et al., 1997  ), and phosphacan binds with high affinity ( Kd ~2 nM) to native TN-R (Milev et al., 1998  ).	bind
32572	1	9268	6	NULL	NULL	0	NULL	phosphacan	NULL		bind	NULL	high affinity			TN-R	NULL	native			NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_11_4245_s_45	10341229	A brain-derived chondroitin sulfate proteoglycan related to phosphacan has been isolated by affinity to a recombinant amino-terminal EGF domain of TN-R (Xiao et al., 1997  ), and phosphacan binds with high affinity ( Kd ~2 nM) to native TN-R (Milev et al., 1998  ).	bind
32573	2	9268	6	NULL	NULL	0	NULL	chondroitin sulfate proteoglycan	NULL	brain-derived	is related to	NULL				phosphacan	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_11_4245_s_45	10341229	A brain-derived chondroitin sulfate proteoglycan related to phosphacan has been isolated by affinity to a recombinant amino-terminal EGF domain of TN-R (Xiao et al., 1997  ), and phosphacan binds with high affinity ( Kd ~2 nM) to native TN-R (Milev et al., 1998  ).	bind
32574	3	9268	6	NULL	NULL	0	NULL	chondroitin sulfate proteoglycan	NULL	brain-derived	has affinity for	NULL				TN-R	NULL	recombinant	amino-terminal EGF domain		NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_11_4245_s_45	10341229	A brain-derived chondroitin sulfate proteoglycan related to phosphacan has been isolated by affinity to a recombinant amino-terminal EGF domain of TN-R (Xiao et al., 1997  ), and phosphacan binds with high affinity ( Kd ~2 nM) to native TN-R (Milev et al., 1998  ).	bind
39936	1	9269	5	13	NULL	NULL	NULL	small glutamine-rich tetratricopeptide repeat-containing protein	GP	brain-specific isoform	bind					Hsc70	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_40_38376_s_1	12878599	A brain-specific isoform of small glutamine-rich tetratricopeptide repeat-containing protein binds to Hsc70 and the cysteine string protein.	bind
39937	2	9269	5	13	NULL	NULL	NULL	small glutamine-rich tetratricopeptide repeat-containing protein	GP	brain-specific isoform	bind					cysteine string protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_40_38376_s_1	12878599	A brain-specific isoform of small glutamine-rich tetratricopeptide repeat-containing protein binds to Hsc70 and the cysteine string protein.	bind
32575	1	9269	6	NULL	NULL	0	NULL	small glutamine-rich tetratricopeptide repeat-containing protein	NULL	brain-specific isoform	bind	NULL				Hsc70	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_40_38376_s_1	12878599	A brain-specific isoform of small glutamine-rich tetratricopeptide repeat-containing protein binds to Hsc70 and the cysteine string protein.	bind
32576	2	9269	6	NULL	NULL	0	NULL	small glutamine-rich tetratricopeptide repeat-containing protein	NULL	brain-specific isoform	bind	NULL				cysteine string protein	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_40_38376_s_1	12878599	A brain-specific isoform of small glutamine-rich tetratricopeptide repeat-containing protein binds to Hsc70 and the cysteine string protein.	bind
39938	1	9270	5	13	NULL	NULL	NULL	guanine nucleotides	NucleicAcid		bind					RF3	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_22_2_175_s_124	12514123	A breakthrough in our understanding of RF3 function occurred when   et al remeasured the binding of guanine nucleotides to this G protein.	bind
39939	2	9270	5	13	NULL	NULL	NULL	RF3	GP		is a type of					G protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_22_2_175_s_124	12514123	A breakthrough in our understanding of RF3 function occurred when   et al remeasured the binding of guanine nucleotides to this G protein.	bind
32577	1	9270	6	10	NULL	0	NULL	guanine nucleotides	NULL		bind	NULL				RF3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_embo_22_2_175_s_124	12514123	A breakthrough in our understanding of RF3 function occurred when   et al remeasured the binding of guanine nucleotides to this G protein.	bind
48085	2	9270	6	10	NULL	0	NULL	RF3	NULL		is a type of	NULL				G protein	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_22_2_175_s_124	12514123	A breakthrough in our understanding of RF3 function occurred when   et al remeasured the binding of guanine nucleotides to this G protein.	bind
40676	1	9272	5	13	NULL	NULL	NULL	BR	Chemical		bind					HSA	GP	native			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1523_2_147_s_121	11042378	A brief (1 min) irradiation of BR bound to native HSA under white fluorescent light, produced only little change in the magnitude of both positive and negative CDCEs (  Fig. 3A).	bind
57865	2	9272	5	13	NULL	NULL	NULL	CDCE	ResearchActivity		change					magnitude	QuantityOrMeasure				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1523_2_147_s_121	11042378	A brief (1 min) irradiation of BR bound to native HSA under white fluorescent light, produced only little change in the magnitude of both positive and negative CDCEs (  Fig. 3A).	bind
57866	3	9272	5	13	NULL	NULL	NULL	statement 1	Process		produced					statement 2	Process	little change in			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1523_2_147_s_121	11042378	A brief (1 min) irradiation of BR bound to native HSA under white fluorescent light, produced only little change in the magnitude of both positive and negative CDCEs (  Fig. 3A).	bind
32578	1	9272	6	NULL	NULL	0	NULL	BR	NULL		bind	NULL				HSA	NULL	native			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1523_2_147_s_121	11042378	A brief (1 min) irradiation of BR bound to native HSA under white fluorescent light, produced only little change in the magnitude of both positive and negative CDCEs (  Fig. 3A).	bind
32579	2	9272	6	NULL	NULL	0	NULL	CDCE	NULL		change	NULL				magnitude	NULL				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1523_2_147_s_121	11042378	A brief (1 min) irradiation of BR bound to native HSA under white fluorescent light, produced only little change in the magnitude of both positive and negative CDCEs (  Fig. 3A).	bind
40523	3	9272	6	NULL	NULL	0	NULL	statement 1	NULL		produced	NULL				statement 2	NULL	little change in			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1523_2_147_s_121	11042378	A brief (1 min) irradiation of BR bound to native HSA under white fluorescent light, produced only little change in the magnitude of both positive and negative CDCEs (  Fig. 3A).	bind
40052	3	9273	5	13	NULL	NULL	NULL	PCA	Chemical		disrupt		strongly			statement 1	Process	formation of			NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_67_8_3530_s_274	11472929	A brief survey of the effects of other aromatic compounds on CbaR binding identified PCA as a strong disrupter of the CbaR-P cbaA complex (Fig.  4F), suggesting that CbaR evolved so that it responds to both 3CBA, the substrate of the  cba pathway, and at least one downstream metabolite.	bind
40054	2	9273	5	13	NULL	NULL	NULL	PCA	Chemical		is a type of					aromatic compound	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_67_8_3530_s_274	11472929	A brief survey of the effects of other aromatic compounds on CbaR binding identified PCA as a strong disrupter of the CbaR-P cbaA complex (Fig.  4F), suggesting that CbaR evolved so that it responds to both 3CBA, the substrate of the  cba pathway, and at least one downstream metabolite.	bind
40057	4	9273	5	13	NULL	NULL	NULL	3CBA	Chemical		substrate of					cba pathway	Process				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_67_8_3530_s_274	11472929	A brief survey of the effects of other aromatic compounds on CbaR binding identified PCA as a strong disrupter of the CbaR-P cbaA complex (Fig.  4F), suggesting that CbaR evolved so that it responds to both 3CBA, the substrate of the  cba pathway, and at least one downstream metabolite.	bind
40058	5	9273	5	13	NULL	NULL	NULL	CbaR	GP		respond to					3CBA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_67_8_3530_s_274	11472929	A brief survey of the effects of other aromatic compounds on CbaR binding identified PCA as a strong disrupter of the CbaR-P cbaA complex (Fig.  4F), suggesting that CbaR evolved so that it responds to both 3CBA, the substrate of the  cba pathway, and at least one downstream metabolite.	bind
48086	1	9273	5	13	NULL	NULL	NULL	CbaR	GP		complex with					P cbaA	GP				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_67_8_3530_s_274	11472929	A brief survey of the effects of other aromatic compounds on CbaR binding identified PCA as a strong disrupter of the CbaR-P cbaA complex (Fig.  4F), suggesting that CbaR evolved so that it responds to both 3CBA, the substrate of the  cba pathway, and at least one downstream metabolite.	bind
32845	4	9273	6	10	NULL	0	NULL	PCA			disrupts		strongly			statement 1		formation of			NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_67_8_3530_s_274	11472929	A brief survey of the effects of other aromatic compounds on CbaR binding identified PCA as a strong disrupter of the CbaR-P cbaA complex (Fig.  4F), suggesting that CbaR evolved so that it responds to both 3CBA, the substrate of the  cba pathway, and at least one downstream metabolite.	bind
32847	2	9273	6	NULL	NULL	0	NULL	CbaR	NULL		responds to	NULL				3CBA	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_67_8_3530_s_274	11472929	A brief survey of the effects of other aromatic compounds on CbaR binding identified PCA as a strong disrupter of the CbaR-P cbaA complex (Fig.  4F), suggesting that CbaR evolved so that it responds to both 3CBA, the substrate of the  cba pathway, and at least one downstream metabolite.	bind
32850	3	9273	6	10	NULL	0	NULL	3CBA	NULL		substrate of	NULL				 cba pathway	NULL				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_67_8_3530_s_274	11472929	A brief survey of the effects of other aromatic compounds on CbaR binding identified PCA as a strong disrupter of the CbaR-P cbaA complex (Fig.  4F), suggesting that CbaR evolved so that it responds to both 3CBA, the substrate of the  cba pathway, and at least one downstream metabolite.	bind
48087	1	9273	6	10	NULL	0	NULL	CbaR	NULL		complex with	NULL				P cbaA	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_67_8_3530_s_274	11472929	A brief survey of the effects of other aromatic compounds on CbaR binding identified PCA as a strong disrupter of the CbaR-P cbaA complex (Fig.  4F), suggesting that CbaR evolved so that it responds to both 3CBA, the substrate of the  cba pathway, and at least one downstream metabolite.	bind
48088	5	9273	6	10	NULL	0	NULL	PCA	NULL		is a type of	NULL				aromatic compound	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_67_8_3530_s_274	11472929	A brief survey of the effects of other aromatic compounds on CbaR binding identified PCA as a strong disrupter of the CbaR-P cbaA complex (Fig.  4F), suggesting that CbaR evolved so that it responds to both 3CBA, the substrate of the  cba pathway, and at least one downstream metabolite.	bind
39944	1	9274	5	13	NULL	NULL	NULL	BrlA-like protein	GP		bind					ech42	NucleicAcid			promoter	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_218_2_259_s_66	12586401	A BrlA-like protein binds to the  ech42 promoter under carbon starvation in vitro	bind
39945	2	9274	5	13	NULL	NULL	NULL	statement 1	Process		occurs under					carbon 	Chemical	starvation of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_218_2_259_s_66	12586401	A BrlA-like protein binds to the  ech42 promoter under carbon starvation in vitro	bind
32580	1	9274	6	NULL	NULL	0	NULL	BrlA-like protein	NULL		bind	NULL				ech42	NULL			promoter	NULL	in vitro	0	NULL	NULL	NULL	gw60_femsmicrobiollett_218_2_259_s_66	12586401	A BrlA-like protein binds to the  ech42 promoter under carbon starvation in vitro	bind
32581	2	9274	6	10	NULL	0	NULL	statement 1			occurs under					carbon 		starvation of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_218_2_259_s_66	12586401	A BrlA-like protein binds to the  ech42 promoter under carbon starvation in vitro	bind
40059	1	9278	5	13	NULL	NULL	NULL	C-C chemokine receptor	GP		bind					C-C chemokine family	GP	multiple members of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_18_10439_s_24	7737978	A C-C chemokine receptor, which  binds multiple members of the C-C chemokine family and two monocyte  chemotactic protein-1 receptors have also been cloned  ( 9,  10) .	bind
40060	2	9278	5	13	NULL	NULL	NULL	C-C chemokine receptor	GP		bind					monocyte chemotactic protein-1 receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_18_10439_s_24	7737978	A C-C chemokine receptor, which  binds multiple members of the C-C chemokine family and two monocyte  chemotactic protein-1 receptors have also been cloned  ( 9,  10) .	bind
32583	1	9278	6	NULL	NULL	0	NULL	C-C chemokine receptor	NULL		bind	NULL				C-C chemokine family	NULL	multiple members of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_18_10439_s_24	7737978	A C-C chemokine receptor, which  binds multiple members of the C-C chemokine family and two monocyte  chemotactic protein-1 receptors have also been cloned  ( 9,  10) .	bind
32584	2	9278	6	10	NULL	0	NULL	C-C chemokine receptor			bind					monocyte chemotactic protein-1 receptor					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_18_10439_s_24	7737978	A C-C chemokine receptor, which  binds multiple members of the C-C chemokine family and two monocyte  chemotactic protein-1 receptors have also been cloned  ( 9,  10) .	bind
40064	1	9279	5	13	NULL	NULL	NULL	c-FosJunD heterodimer	GP		bind					GST-BAF60a	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_4_2852_s_91	11053448	A c-FosunD heterodimer bound with GST-BAF60a, but the binding was less than that observed with c-Fos alone (Fig.  2 B), suggesting that dimerization of c-Fos and JunD did not appreciably contribute to BAF60a binding.	bind
40066	2	9279	5	13	NULL	NULL	NULL	c-Fos	GP		bind					GST-BAF60a	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_4_2852_s_91	11053448	A c-FosunD heterodimer bound with GST-BAF60a, but the binding was less than that observed with c-Fos alone (Fig.  2 B), suggesting that dimerization of c-Fos and JunD did not appreciably contribute to BAF60a binding.	bind
40068	3	9279	5	13	NULL	NULL	NULL	statement 1	Process	affinity of	less than					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_4_2852_s_91	11053448	A c-FosunD heterodimer bound with GST-BAF60a, but the binding was less than that observed with c-Fos alone (Fig.  2 B), suggesting that dimerization of c-Fos and JunD did not appreciably contribute to BAF60a binding.	bind
40074	4	9279	5	13	NULL	NULL	NULL	c-Fos	GP		dimerize with					JunD	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_4_2852_s_91	11053448	A c-FosunD heterodimer bound with GST-BAF60a, but the binding was less than that observed with c-Fos alone (Fig.  2 B), suggesting that dimerization of c-Fos and JunD did not appreciably contribute to BAF60a binding.	bind
40075	5	9279	5	13	NULL	NULL	NULL	statement 4	Process		does not contribute to		appreciably			BAF60a	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_4_2852_s_91	11053448	A c-FosunD heterodimer bound with GST-BAF60a, but the binding was less than that observed with c-Fos alone (Fig.  2 B), suggesting that dimerization of c-Fos and JunD did not appreciably contribute to BAF60a binding.	bind
32585	1	9279	6	NULL	NULL	0	NULL	c-FosunD heterodimer	NULL		bind	NULL				GST-BAF60a	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_4_2852_s_91	11053448	A c-FosunD heterodimer bound with GST-BAF60a, but the binding was less than that observed with c-Fos alone (Fig.  2 B), suggesting that dimerization of c-Fos and JunD did not appreciably contribute to BAF60a binding.	bind
32586	2	9279	6	NULL	NULL	0	NULL	c-Fos	NULL		bind	NULL				GST-BAF60a	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_4_2852_s_91	11053448	A c-FosunD heterodimer bound with GST-BAF60a, but the binding was less than that observed with c-Fos alone (Fig.  2 B), suggesting that dimerization of c-Fos and JunD did not appreciably contribute to BAF60a binding.	bind
32587	3	9279	6	NULL	NULL	0	NULL	statement 1	NULL	affinity of	is less than	NULL				statement 2	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_4_2852_s_91	11053448	A c-FosunD heterodimer bound with GST-BAF60a, but the binding was less than that observed with c-Fos alone (Fig.  2 B), suggesting that dimerization of c-Fos and JunD did not appreciably contribute to BAF60a binding.	bind
32588	4	9279	6	NULL	NULL	0	NULL	c-Fos	NULL		dimerizes with	NULL				JunD	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_4_2852_s_91	11053448	A c-FosunD heterodimer bound with GST-BAF60a, but the binding was less than that observed with c-Fos alone (Fig.  2 B), suggesting that dimerization of c-Fos and JunD did not appreciably contribute to BAF60a binding.	bind
32589	5	9279	6	NULL	NULL	0	NULL	statement 4	NULL		did not contribute to	NULL				BAF60a	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_4_2852_s_91	11053448	A c-FosunD heterodimer bound with GST-BAF60a, but the binding was less than that observed with c-Fos alone (Fig.  2 B), suggesting that dimerization of c-Fos and JunD did not appreciably contribute to BAF60a binding.	bind
40079	1	9280	5	13	NULL	NULL	NULL	MarR	GP	deletion mutant	reduce			C-terminal 18 amino acid 		MarR	GP	binding properties of			NULL	clinical isolate of Escherichia coli 	NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_4_671_s_1443	12456787	A C-terminal 18 amino acid deletion in MarR in a clinical isolate of  Escherichia coli reduces MarR binding properties and increases the MIC of ciprofloxacin.	bind
40083	2	9280	5	13	NULL	NULL	NULL	statement 1	Process		increase					ciprofloxacin	Chemical	MIC of			NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_4_671_s_1443	12456787	A C-terminal 18 amino acid deletion in MarR in a clinical isolate of  Escherichia coli reduces MarR binding properties and increases the MIC of ciprofloxacin.	bind
32853	1	9280	6	NULL	NULL	0	NULL	MarR	NULL	deletion of	reduces	NULL		C-terminal 18 amino acid		MarR	NULL	binding properties of			NULL	clinical isolate of Escherichia coli 	NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_4_671_s_1443	12456787	A C-terminal 18 amino acid deletion in MarR in a clinical isolate of  Escherichia coli reduces MarR binding properties and increases the MIC of ciprofloxacin.	bind
32856	2	9280	6	NULL	NULL	0	NULL	MarR	NULL	deletion of	increases	NULL		C-terminal 18 amino acid		ciprofloxacin	NULL	MIC of 			NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_4_671_s_1443	12456787	A C-terminal 18 amino acid deletion in MarR in a clinical isolate of  Escherichia coli reduces MarR binding properties and increases the MIC of ciprofloxacin.	bind
40380	2	9282	5	13	NULL	NULL	NULL	ELL sequences	GP		is implicated in					leukemogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_17_7803_s_119	16107725	A C-terminal deletion removed the last 300 amino acids of dELL, which contain homology to the ELL sequences implicated in leukemogenesis ( ,  ), to the minimal p53 binding sequence of ELL ( ), and to the ZO-1 binding domain of occludin.	bind
40382	1	9282	5	13	NULL	NULL	NULL	dELL	GP		is homologous to			last 300 amino acids		ELL sequences	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_17_7803_s_119	16107725	A C-terminal deletion removed the last 300 amino acids of dELL, which contain homology to the ELL sequences implicated in leukemogenesis ( ,  ), to the minimal p53 binding sequence of ELL ( ), and to the ZO-1 binding domain of occludin.	bind
40383	3	9282	5	13	NULL	NULL	NULL	dELL	GP		is homologous to			last 300 amino acids		ELL	GP		p53 binding sequence		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_17_7803_s_119	16107725	A C-terminal deletion removed the last 300 amino acids of dELL, which contain homology to the ELL sequences implicated in leukemogenesis ( ,  ), to the minimal p53 binding sequence of ELL ( ), and to the ZO-1 binding domain of occludin.	bind
40384	4	9282	5	13	NULL	NULL	NULL	dELL	GP		is homologous to			last 300 amino acids		occludin	GP		ZO-1 binding domain		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_17_7803_s_119	16107725	A C-terminal deletion removed the last 300 amino acids of dELL, which contain homology to the ELL sequences implicated in leukemogenesis ( ,  ), to the minimal p53 binding sequence of ELL ( ), and to the ZO-1 binding domain of occludin.	bind
32859	1	9282	6	NULL	NULL	0	NULL	ELL sequences	NULL		are implicated in	NULL				leukemogenesis	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_17_7803_s_119	16107725	A C-terminal deletion removed the last 300 amino acids of dELL, which contain homology to the ELL sequences implicated in leukemogenesis ( ,  ), to the minimal p53 binding sequence of ELL ( ), and to the ZO-1 binding domain of occludin.	bind
32860	2	9282	6	10	NULL	0	NULL	dELL			is homologous to			last 300 amino acids		ELL sequences					NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_17_7803_s_119	16107725	A C-terminal deletion removed the last 300 amino acids of dELL, which contain homology to the ELL sequences implicated in leukemogenesis ( ,  ), to the minimal p53 binding sequence of ELL ( ), and to the ZO-1 binding domain of occludin.	bind
48089	3	9282	6	10	NULL	0	NULL	dELL	NULL		is homologous to	NULL		last 300 amino acids		ELL	NULL		 p53 binding sequence		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_17_7803_s_119	16107725	A C-terminal deletion removed the last 300 amino acids of dELL, which contain homology to the ELL sequences implicated in leukemogenesis ( ,  ), to the minimal p53 binding sequence of ELL ( ), and to the ZO-1 binding domain of occludin.	bind
48090	4	9282	6	10	NULL	0	NULL	dELL	NULL		is homologous to	NULL		last 300 amino acids		occludin	NULL		ZO-1 binding domain		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_17_7803_s_119	16107725	A C-terminal deletion removed the last 300 amino acids of dELL, which contain homology to the ELL sequences implicated in leukemogenesis ( ,  ), to the minimal p53 binding sequence of ELL ( ), and to the ZO-1 binding domain of occludin.	bind
40087	1	9283	5	13	NULL	NULL	NULL	K cyclin-cdk6	GP		phosphorylate					p27Kip1	GP		C-terminal fragment		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_3_654_s_107	9927425	A C-terminal fragment of p27Kip1 synthesized as a GST fusion protein in bacteria was bound to glutathione-Sepharose beads and phosphorylated by either K cyclin-cdk6	bind
48091	2	9283	5	13	NULL	NULL	NULL	p27Kip1	GP		is a type of					GST fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_3_654_s_107	9927425	A C-terminal fragment of p27Kip1 synthesized as a GST fusion protein in bacteria was bound to glutathione-Sepharose beads and phosphorylated by either K cyclin-cdk6	bind
32590	1	9283	6	10	NULL	0	NULL	K cyclin-cdk6	NULL		phosphorylates	NULL				p27Kip1	NULL		C-terminal fragment		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_3_654_s_107	9927425	A C-terminal fragment of p27Kip1 synthesized as a GST fusion protein in bacteria was bound to glutathione-Sepharose beads and phosphorylated by either K cyclin-cdk6	bind
48092	2	9283	6	10	NULL	0	NULL	p27Kip1	NULL		is a type of	NULL				GST fusion protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_3_654_s_107	9927425	A C-terminal fragment of p27Kip1 synthesized as a GST fusion protein in bacteria was bound to glutathione-Sepharose beads and phosphorylated by either K cyclin-cdk6	bind
40088	1	9284	5	13	NULL	NULL	NULL	 papillomavirus E1 protein	GP	human	bind			C-terminal helicase domain		E2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_1_149_s_427	10949036	A C-terminal helicase domain of the human papillomavirus E1 protein binds E2 and the DNA polymerase  -primase p68 subunit.	bind
40089	2	9284	5	13	NULL	NULL	NULL	 papillomavirus E1 protein	GP	human	bind			C-terminal helicase domain		DNA polymerase -primase	GP		p68 subunit		NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_1_149_s_427	10949036	A C-terminal helicase domain of the human papillomavirus E1 protein binds E2 and the DNA polymerase  -primase p68 subunit.	bind
32591	1	9284	6	NULL	NULL	0	NULL	papillomavirus E1 protein	NULL	human	bind	NULL		C-terminal helicase domain		E2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_6_1_149_s_427	10949036	A C-terminal helicase domain of the human papillomavirus E1 protein binds E2 and the DNA polymerase  -primase p68 subunit.	bind
32592	2	9284	6	10	NULL	0	NULL	papillomavirus E1 protein	NULL	human	bind	NULL		C-terminal helicase domain		DNA polymerase -primase 	NULL		p68 subunit		NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_1_149_s_427	10949036	A C-terminal helicase domain of the human papillomavirus E1 protein binds E2 and the DNA polymerase  -primase p68 subunit.	bind
40090	1	9286	5	13	NULL	NULL	NULL				bind			C-terminal IQ domain		calmodulin	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_blood_108_2_16569770_s_4	16569770	A C-terminal IQ domain binds calmodulin in the absence of calcium, and  conserved PKC phosphorylation motifs are targets of concanavalin A (ConA)-  or PMA/ionomycin-induced PKC activation.	bind
40091	2	9286	5	13	NULL	NULL	NULL	statement 1	Process		in the absence of					calcium	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_blood_108_2_16569770_s_4	16569770	A C-terminal IQ domain binds calmodulin in the absence of calcium, and  conserved PKC phosphorylation motifs are targets of concanavalin A (ConA)-  or PMA/ionomycin-induced PKC activation.	bind
40092	3	9286	5	13	NULL	NULL	NULL	ConA	GP		induce					PKC	GP	activation of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_blood_108_2_16569770_s_4	16569770	A C-terminal IQ domain binds calmodulin in the absence of calcium, and  conserved PKC phosphorylation motifs are targets of concanavalin A (ConA)-  or PMA/ionomycin-induced PKC activation.	bind
40093	4	9286	5	13	NULL	NULL	NULL	PMA/ionomycin	Chemical		induce					PKC	GP	activation of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_blood_108_2_16569770_s_4	16569770	A C-terminal IQ domain binds calmodulin in the absence of calcium, and  conserved PKC phosphorylation motifs are targets of concanavalin A (ConA)-  or PMA/ionomycin-induced PKC activation.	bind
40094	5	9286	5	13	NULL	NULL	NULL	PKC	GP		are targets of			conserved phosphorylation motifs		statement 3	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_blood_108_2_16569770_s_4	16569770	A C-terminal IQ domain binds calmodulin in the absence of calcium, and  conserved PKC phosphorylation motifs are targets of concanavalin A (ConA)-  or PMA/ionomycin-induced PKC activation.	bind
48093	6	9286	5	13	NULL	NULL	NULL	ConA	GP		is					concanavalin A	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_blood_108_2_16569770_s_4	16569770	A C-terminal IQ domain binds calmodulin in the absence of calcium, and  conserved PKC phosphorylation motifs are targets of concanavalin A (ConA)-  or PMA/ionomycin-induced PKC activation.	bind
57919	7	9286	5	13	NULL	NULL	NULL	PKC	GP		are targets of			conserved phosphorylation motifs		statement 4	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_blood_108_2_16569770_s_4	16569770	A C-terminal IQ domain binds calmodulin in the absence of calcium, and  conserved PKC phosphorylation motifs are targets of concanavalin A (ConA)-  or PMA/ionomycin-induced PKC activation.	bind
32593	1	9286	6	NULL	NULL	0	NULL		NULL		bind	NULL		C-terminal IQ domain		calmodulin	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_blood_108_2_16569770_s_4	16569770	A C-terminal IQ domain binds calmodulin in the absence of calcium, and  conserved PKC phosphorylation motifs are targets of concanavalin A (ConA)-  or PMA/ionomycin-induced PKC activation.	bind
32594	2	9286	6	NULL	NULL	0	NULL	statement 1	NULL		occurs in absence of	NULL				calcium	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_blood_108_2_16569770_s_4	16569770	A C-terminal IQ domain binds calmodulin in the absence of calcium, and  conserved PKC phosphorylation motifs are targets of concanavalin A (ConA)-  or PMA/ionomycin-induced PKC activation.	bind
32861	3	9286	6	NULL	NULL	0	NULL	ConA	NULL		is	NULL				concanavalin A	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_blood_108_2_16569770_s_4	16569770	A C-terminal IQ domain binds calmodulin in the absence of calcium, and  conserved PKC phosphorylation motifs are targets of concanavalin A (ConA)-  or PMA/ionomycin-induced PKC activation.	bind
32862	4	9286	6	NULL	NULL	0	NULL	ConA	NULL		induces	NULL				PKC	NULL	activation of			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_blood_108_2_16569770_s_4	16569770	A C-terminal IQ domain binds calmodulin in the absence of calcium, and  conserved PKC phosphorylation motifs are targets of concanavalin A (ConA)-  or PMA/ionomycin-induced PKC activation.	bind
32863	5	9286	6	NULL	NULL	0	NULL	PMA/ionomycin	NULL		induces	NULL				PKC	NULL	activation of			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_blood_108_2_16569770_s_4	16569770	A C-terminal IQ domain binds calmodulin in the absence of calcium, and  conserved PKC phosphorylation motifs are targets of concanavalin A (ConA)-  or PMA/ionomycin-induced PKC activation.	bind
32864	6	9286	6	NULL	NULL	0	NULL		NULL	conserved	are targets of	NULL		PKC phosphorylation motif		statement 4	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_blood_108_2_16569770_s_4	16569770	A C-terminal IQ domain binds calmodulin in the absence of calcium, and  conserved PKC phosphorylation motifs are targets of concanavalin A (ConA)-  or PMA/ionomycin-induced PKC activation.	bind
32865	7	9286	6	NULL	NULL	0	NULL		NULL	conserved	are targets of	NULL		PKC phosphorylation motif		statement 5	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_blood_108_2_16569770_s_4	16569770	A C-terminal IQ domain binds calmodulin in the absence of calcium, and  conserved PKC phosphorylation motifs are targets of concanavalin A (ConA)-  or PMA/ionomycin-induced PKC activation.	bind
40095	1	9287	5	13	NULL	NULL	NULL	Mst27p	GP		bind		directly	C-terminal KKXX motif		COPI complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_8_3097_s_6	12925749	A C-terminal KKXX motif of Mst27p that allows direct  binding to the COPI complex is crucial for its suppression ability.	bind
40096	2	9287	5	13	NULL	NULL	NULL	Mst27p	GP		is required for		crucial	C-terminal KKXX motif		Mst27p	GP	suppression ability of			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_8_3097_s_6	12925749	A C-terminal KKXX motif of Mst27p that allows direct  binding to the COPI complex is crucial for its suppression ability.	bind
32595	1	9287	6	NULL	NULL	0	NULL	Mst27p	NULL		bind	NULL	direct	C-terminal KKXX motif		COPI complex	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_8_3097_s_6	12925749	A C-terminal KKXX motif of Mst27p that allows direct  binding to the COPI complex is crucial for its suppression ability.	bind
32629	2	9287	6	10	NULL	0	NULL	Mst27p			is crucial for			C-terminal KKXX motif		Mst27p		 suppression ability of			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_8_3097_s_6	12925749	A C-terminal KKXX motif of Mst27p that allows direct  binding to the COPI complex is crucial for its suppression ability.	bind
40097	2	9290	5	13	NULL	NULL	NULL	PDK3	GP	truncated	abolishes			C-terminal delta392 406		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_10_1763_s_223	15861126	A C-terminal truncation (delta392 406) of PDK3 abolishes L2 binding to PDK3 as determined by ITC ( Figure 3).	bind
40098	1	9290	5	13	NULL	NULL	NULL	L2	GP		bind					PDK3	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_10_1763_s_223	15861126	A C-terminal truncation (delta392 406) of PDK3 abolishes L2 binding to PDK3 as determined by ITC ( Figure 3).	bind
32632	1	9290	6	NULL	NULL	0	NULL	L2	NULL		bind	NULL				PDK3	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_24_10_1763_s_223	15861126	A C-terminal truncation (delta392 406) of PDK3 abolishes L2 binding to PDK3 as determined by ITC ( Figure 3).	bind
32633	2	9290	6	10	NULL	0	NULL	PDK3		truncated	abolishes			C-terminal delta392 406		statement 1					NULL		NULL	NULL	NULL	NULL	gw70_embo_24_10_1763_s_223	15861126	A C-terminal truncation (delta392 406) of PDK3 abolishes L2 binding to PDK3 as determined by ITC ( Figure 3).	bind
40102	1	9292	5	13	NULL	NULL	NULL	IKKgamma	GP	 truncated	lacks			C-terminal					LZ		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4547_s_43	10373503	A C-terminally truncated version of IKKgamma lacking the LZ can still bind IKKalpha-IKKbeta heterodimers, but once expressed, it prevents IKK activation by a number of stimuli, including TNF and IL-1 ( 33).	bind
40103	2	9292	5	13	NULL	NULL	NULL	statement 1	GP		bind					IKKalpha-IKKbeta heterodimers	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4547_s_43	10373503	A C-terminally truncated version of IKKgamma lacking the LZ can still bind IKKalpha-IKKbeta heterodimers, but once expressed, it prevents IKK activation by a number of stimuli, including TNF and IL-1 ( 33).	bind
40104	3	9292	5	13	NULL	NULL	NULL	TNF	GP		stimulates					IKK	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4547_s_43	10373503	A C-terminally truncated version of IKKgamma lacking the LZ can still bind IKKalpha-IKKbeta heterodimers, but once expressed, it prevents IKK activation by a number of stimuli, including TNF and IL-1 ( 33).	bind
40105	4	9292	5	13	NULL	NULL	NULL	IL-1	GP		stimulates					IKK	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4547_s_43	10373503	A C-terminally truncated version of IKKgamma lacking the LZ can still bind IKKalpha-IKKbeta heterodimers, but once expressed, it prevents IKK activation by a number of stimuli, including TNF and IL-1 ( 33).	bind
40106	5	9292	5	13	NULL	NULL	NULL	IKKgamma	GP	expression of;;truncated	prevents			C-terminal		statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4547_s_43	10373503	A C-terminally truncated version of IKKgamma lacking the LZ can still bind IKKalpha-IKKbeta heterodimers, but once expressed, it prevents IKK activation by a number of stimuli, including TNF and IL-1 ( 33).	bind
40107	6	9292	5	13	NULL	NULL	NULL	IKKgamma	GP	expression of;;truncated	prevents			C-terminal		statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4547_s_43	10373503	A C-terminally truncated version of IKKgamma lacking the LZ can still bind IKKalpha-IKKbeta heterodimers, but once expressed, it prevents IKK activation by a number of stimuli, including TNF and IL-1 ( 33).	bind
32638	1	9292	6	NULL	NULL	0	NULL	IKKgamma	NULL	truncated	bind	NULL		C-terminal		IKKalpha-IKKbeta heterodimers	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_7_4547_s_43	10373503	A C-terminally truncated version of IKKgamma lacking the LZ can still bind IKKalpha-IKKbeta heterodimers, but once expressed, it prevents IKK activation by a number of stimuli, including TNF and IL-1 ( 33).	bind
32866	2	9292	6	NULL	NULL	0	NULL	TNF	NULL		stimulates	NULL				IKK	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_7_4547_s_43	10373503	A C-terminally truncated version of IKKgamma lacking the LZ can still bind IKKalpha-IKKbeta heterodimers, but once expressed, it prevents IKK activation by a number of stimuli, including TNF and IL-1 ( 33).	bind
32867	3	9292	6	NULL	NULL	0	NULL	IL-1	NULL		stimulates	NULL				IKK	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_7_4547_s_43	10373503	A C-terminally truncated version of IKKgamma lacking the LZ can still bind IKKalpha-IKKbeta heterodimers, but once expressed, it prevents IKK activation by a number of stimuli, including TNF and IL-1 ( 33).	bind
32868	4	9292	6	NULL	NULL	0	NULL	IKKgamma	NULL	expression of;; truncated	prevents	NULL		C-terminal		statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_7_4547_s_43	10373503	A C-terminally truncated version of IKKgamma lacking the LZ can still bind IKKalpha-IKKbeta heterodimers, but once expressed, it prevents IKK activation by a number of stimuli, including TNF and IL-1 ( 33).	bind
32869	5	9292	6	NULL	NULL	0	NULL	IKKgamma	NULL	expression of;; truncated	prevents	NULL		C-terminal		statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_7_4547_s_43	10373503	A C-terminally truncated version of IKKgamma lacking the LZ can still bind IKKalpha-IKKbeta heterodimers, but once expressed, it prevents IKK activation by a number of stimuli, including TNF and IL-1 ( 33).	bind
48094	6	9292	6	10	NULL	0	NULL	IKKgamma	NULL	truncated	lacks	NULL		C-terminal			NULL		LZ		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_7_4547_s_43	10373503	A C-terminally truncated version of IKKgamma lacking the LZ can still bind IKKalpha-IKKbeta heterodimers, but once expressed, it prevents IKK activation by a number of stimuli, including TNF and IL-1 ( 33).	bind
40111	1	9293	5	13	NULL	NULL	NULL	C/EBP-like transcription factor	GP		bind									X2 region of early promoters	NULL		NULL	NULL	NULL	NULL	gw70_insectbiochemmolbiol_33_5_525_s_211	12706632	A C/EBP-like transcription factor binds to the X2 region of early promoters	bind
32639	1	9293	6	NULL	NULL	0	NULL	C/EBP-like transcription factor	NULL		bind	NULL					NULL			X2 region of promoter	NULL		0	NULL	NULL	NULL	gw70_insectbiochemmolbiol_33_5_525_s_211	12706632	A C/EBP-like transcription factor binds to the X2 region of early promoters	bind
40112	1	9294	5	13	NULL	NULL	NULL	metalloid	Chemical		bind		high affinity			ArsA	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_15_9925_s_26	16467301	A C113A/C422A mutation introduced into ArsA was found to eliminate high affinity metalloid binding to ArsA.	bind
40113	2	9294	5	13	NULL	NULL	NULL	ArsA	GP	mutant	prevents			C113A/C422A		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_15_9925_s_26	16467301	A C113A/C422A mutation introduced into ArsA was found to eliminate high affinity metalloid binding to ArsA.	bind
32641	1	9294	6	NULL	NULL	0	NULL	metalloid	NULL		bind	NULL	high affinity			ArsA	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_15_9925_s_26	16467301	A C113A/C422A mutation introduced into ArsA was found to eliminate high affinity metalloid binding to ArsA.	bind
32642	2	9294	6	NULL	NULL	0	NULL	ArsA	NULL	mutant	eliminates	NULL		C113A/C422A		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_15_9925_s_26	16467301	A C113A/C422A mutation introduced into ArsA was found to eliminate high affinity metalloid binding to ArsA.	bind
40114	1	9295	5	13	NULL	NULL	NULL	C3	GP		bind					HbhA	GP				NULL	cell lysates of M. tuberculosis	NULL	NULL	NULL	NULL	gw60_infectimmun_70_12_6751_s_254	12438350	A C3 ligand affinity blotting protocol was previously used by our group to demonstrate binding of C3 to HbhA present in cell lysates of  M. tuberculosis ( 20).	bind
32643	1	9295	6	NULL	NULL	0	NULL	C3	NULL		bind	NULL				HbhA	NULL				NULL	cell lysates of M. tuberculosis	0	NULL	NULL	NULL	gw60_infectimmun_70_12_6751_s_254	12438350	A C3 ligand affinity blotting protocol was previously used by our group to demonstrate binding of C3 to HbhA present in cell lysates of  M. tuberculosis ( 20).	bind
40115	1	9296	5	13	NULL	NULL	NULL	Ca-dependent receptor	GP		resemble					neurexin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_18_16_6113_s_16	9698306	A Ca-dependent receptor that resembles neurexin binds synaptotagmin, a putative Ca sensor (Petrenko et al., 1991  ; Ushkaryov et al., 1992  ); a Ca-independent receptor (CIRL/latrophilin) (Davletov et al., 1996  ; Krasnoperov et al., 1996  ) that resembles members of a family of G-protein-coupled membrane receptors binds to syntaxin, a putative component of the vesicle-docking complex (Bennett and Scheller, 1994  ).	bind
40116	2	9296	5	13	NULL	NULL	NULL	statement 1	GP		bind					synaptotagmin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_18_16_6113_s_16	9698306	A Ca-dependent receptor that resembles neurexin binds synaptotagmin, a putative Ca sensor (Petrenko et al., 1991  ; Ushkaryov et al., 1992  ); a Ca-independent receptor (CIRL/latrophilin) (Davletov et al., 1996  ; Krasnoperov et al., 1996  ) that resembles members of a family of G-protein-coupled membrane receptors binds to syntaxin, a putative component of the vesicle-docking complex (Bennett and Scheller, 1994  ).	bind
40117	3	9296	5	13	NULL	NULL	NULL	synaptotagmin	GP		is a type of					Ca sensor	GP	putative			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_18_16_6113_s_16	9698306	A Ca-dependent receptor that resembles neurexin binds synaptotagmin, a putative Ca sensor (Petrenko et al., 1991  ; Ushkaryov et al., 1992  ); a Ca-independent receptor (CIRL/latrophilin) (Davletov et al., 1996  ; Krasnoperov et al., 1996  ) that resembles members of a family of G-protein-coupled membrane receptors binds to syntaxin, a putative component of the vesicle-docking complex (Bennett and Scheller, 1994  ).	bind
40118	4	9296	5	13	NULL	NULL	NULL	CIRL/latrophilin	GP		resemble					 G-protein-coupled membrane receptors	GP	members of;;family of			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_18_16_6113_s_16	9698306	A Ca-dependent receptor that resembles neurexin binds synaptotagmin, a putative Ca sensor (Petrenko et al., 1991  ; Ushkaryov et al., 1992  ); a Ca-independent receptor (CIRL/latrophilin) (Davletov et al., 1996  ; Krasnoperov et al., 1996  ) that resembles members of a family of G-protein-coupled membrane receptors binds to syntaxin, a putative component of the vesicle-docking complex (Bennett and Scheller, 1994  ).	bind
40119	5	9296	5	13	NULL	NULL	NULL	CIRL/latrophilin	GP		is a type of					Ca-independent receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_18_16_6113_s_16	9698306	A Ca-dependent receptor that resembles neurexin binds synaptotagmin, a putative Ca sensor (Petrenko et al., 1991  ; Ushkaryov et al., 1992  ); a Ca-independent receptor (CIRL/latrophilin) (Davletov et al., 1996  ; Krasnoperov et al., 1996  ) that resembles members of a family of G-protein-coupled membrane receptors binds to syntaxin, a putative component of the vesicle-docking complex (Bennett and Scheller, 1994  ).	bind
40120	6	9296	5	13	NULL	NULL	NULL	CIRL/latrophilin	GP		bind					syntaxin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_18_16_6113_s_16	9698306	A Ca-dependent receptor that resembles neurexin binds synaptotagmin, a putative Ca sensor (Petrenko et al., 1991  ; Ushkaryov et al., 1992  ); a Ca-independent receptor (CIRL/latrophilin) (Davletov et al., 1996  ; Krasnoperov et al., 1996  ) that resembles members of a family of G-protein-coupled membrane receptors binds to syntaxin, a putative component of the vesicle-docking complex (Bennett and Scheller, 1994  ).	bind
40121	7	9296	5	13	NULL	NULL	NULL	syntaxin	GP		is a component of		putative			vesicle-docking complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_18_16_6113_s_16	9698306	A Ca-dependent receptor that resembles neurexin binds synaptotagmin, a putative Ca sensor (Petrenko et al., 1991  ; Ushkaryov et al., 1992  ); a Ca-independent receptor (CIRL/latrophilin) (Davletov et al., 1996  ; Krasnoperov et al., 1996  ) that resembles members of a family of G-protein-coupled membrane receptors binds to syntaxin, a putative component of the vesicle-docking complex (Bennett and Scheller, 1994  ).	bind
32646	1	9296	6	NULL	NULL	0	NULL	Ca-dependent receptor	NULL		resembles	NULL				neurexin	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_18_16_6113_s_16	9698306	A Ca-dependent receptor that resembles neurexin binds synaptotagmin, a putative Ca sensor (Petrenko et al., 1991  ; Ushkaryov et al., 1992  ); a Ca-independent receptor (CIRL/latrophilin) (Davletov et al., 1996  ; Krasnoperov et al., 1996  ) that resembles members of a family of G-protein-coupled membrane receptors binds to syntaxin, a putative component of the vesicle-docking complex (Bennett and Scheller, 1994  ).	bind
32647	2	9296	6	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL				synaptotagmin	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_18_16_6113_s_16	9698306	A Ca-dependent receptor that resembles neurexin binds synaptotagmin, a putative Ca sensor (Petrenko et al., 1991  ; Ushkaryov et al., 1992  ); a Ca-independent receptor (CIRL/latrophilin) (Davletov et al., 1996  ; Krasnoperov et al., 1996  ) that resembles members of a family of G-protein-coupled membrane receptors binds to syntaxin, a putative component of the vesicle-docking complex (Bennett and Scheller, 1994  ).	bind
32649	3	9296	6	NULL	NULL	0	NULL	synaptotagmin	NULL		is a type of	NULL				Ca sensor	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_18_16_6113_s_16	9698306	A Ca-dependent receptor that resembles neurexin binds synaptotagmin, a putative Ca sensor (Petrenko et al., 1991  ; Ushkaryov et al., 1992  ); a Ca-independent receptor (CIRL/latrophilin) (Davletov et al., 1996  ; Krasnoperov et al., 1996  ) that resembles members of a family of G-protein-coupled membrane receptors binds to syntaxin, a putative component of the vesicle-docking complex (Bennett and Scheller, 1994  ).	bind
32650	4	9296	6	NULL	NULL	0	NULL	CIRL/latrophilin	NULL		bind	NULL				syntaxin	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_18_16_6113_s_16	9698306	A Ca-dependent receptor that resembles neurexin binds synaptotagmin, a putative Ca sensor (Petrenko et al., 1991  ; Ushkaryov et al., 1992  ); a Ca-independent receptor (CIRL/latrophilin) (Davletov et al., 1996  ; Krasnoperov et al., 1996  ) that resembles members of a family of G-protein-coupled membrane receptors binds to syntaxin, a putative component of the vesicle-docking complex (Bennett and Scheller, 1994  ).	bind
32651	5	9296	6	NULL	NULL	0	NULL	CIRL/latrophilin	NULL		is a type of	NULL				Ca-independent receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_18_16_6113_s_16	9698306	A Ca-dependent receptor that resembles neurexin binds synaptotagmin, a putative Ca sensor (Petrenko et al., 1991  ; Ushkaryov et al., 1992  ); a Ca-independent receptor (CIRL/latrophilin) (Davletov et al., 1996  ; Krasnoperov et al., 1996  ) that resembles members of a family of G-protein-coupled membrane receptors binds to syntaxin, a putative component of the vesicle-docking complex (Bennett and Scheller, 1994  ).	bind
32652	6	9296	6	10	NULL	0	NULL	CIRL/latrophilin	NULL		resembles	NULL				 G-protein-coupled membrane receptors	NULL	members of ;;family of			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_18_16_6113_s_16	9698306	A Ca-dependent receptor that resembles neurexin binds synaptotagmin, a putative Ca sensor (Petrenko et al., 1991  ; Ushkaryov et al., 1992  ); a Ca-independent receptor (CIRL/latrophilin) (Davletov et al., 1996  ; Krasnoperov et al., 1996  ) that resembles members of a family of G-protein-coupled membrane receptors binds to syntaxin, a putative component of the vesicle-docking complex (Bennett and Scheller, 1994  ).	bind
32653	7	9296	6	NULL	NULL	0	NULL	Syntaxin	NULL		is a component of	NULL	putative			vesicle-docking complex	NULL	 			NULL		0	NULL	NULL	NULL	gw60_jneurosci_18_16_6113_s_16	9698306	A Ca-dependent receptor that resembles neurexin binds synaptotagmin, a putative Ca sensor (Petrenko et al., 1991  ; Ushkaryov et al., 1992  ); a Ca-independent receptor (CIRL/latrophilin) (Davletov et al., 1996  ; Krasnoperov et al., 1996  ) that resembles members of a family of G-protein-coupled membrane receptors binds to syntaxin, a putative component of the vesicle-docking complex (Bennett and Scheller, 1994  ).	bind
40122	1	9297	5	13	NULL	NULL	NULL	EGFC	GP		is a part of		probably	Ca2+-requiring Site in catalytic domain					substrate recognition site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_1855_s_323	11707438	A Ca2+-requiring Site in the EGFC-catalytic Domain Is Probably Part of the Substrate Recognition Site-- Direct measurement of stoichiometry by equilibrium dialysis measurements showed two C6PS binding sites in GDFXa in the presence of Ca2+ and none in the absence of Ca2+	bind
40123	2	9297	5	13	NULL	NULL	NULL	GDFXa	GP		contains								C6PS binding sites		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_1855_s_323	11707438	A Ca2+-requiring Site in the EGFC-catalytic Domain Is Probably Part of the Substrate Recognition Site-- Direct measurement of stoichiometry by equilibrium dialysis measurements showed two C6PS binding sites in GDFXa in the presence of Ca2+ and none in the absence of Ca2+	bind
40124	3	9297	5	13	NULL	NULL	NULL	statement 2	Process		in the presence of					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_1855_s_323	11707438	A Ca2+-requiring Site in the EGFC-catalytic Domain Is Probably Part of the Substrate Recognition Site-- Direct measurement of stoichiometry by equilibrium dialysis measurements showed two C6PS binding sites in GDFXa in the presence of Ca2+ and none in the absence of Ca2+	bind
40125	4	9297	5	13	NULL	NULL	NULL	GDFXa	GP		does not contain								C6PS binding sites		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_1855_s_323	11707438	A Ca2+-requiring Site in the EGFC-catalytic Domain Is Probably Part of the Substrate Recognition Site-- Direct measurement of stoichiometry by equilibrium dialysis measurements showed two C6PS binding sites in GDFXa in the presence of Ca2+ and none in the absence of Ca2+	bind
40126	5	9297	5	13	NULL	NULL	NULL	statement 4	Process		in the absence of					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_1855_s_323	11707438	A Ca2+-requiring Site in the EGFC-catalytic Domain Is Probably Part of the Substrate Recognition Site-- Direct measurement of stoichiometry by equilibrium dialysis measurements showed two C6PS binding sites in GDFXa in the presence of Ca2+ and none in the absence of Ca2+	bind
48095	1	9299	5	13	NULL	NULL	NULL	calcium ion	Chemical		bind					 ADAM33	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_11_2388_s_67	16688218	A calcium ion and a water molecule bound to ADAM33 are represented as green and red  spheres, respectively.	bind
48096	2	9299	5	13	NULL	NULL	NULL	water molecule	Chemical		bind					ADAM33	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_11_2388_s_67	16688218	A calcium ion and a water molecule bound to ADAM33 are represented as green and red  spheres, respectively.	bind
32654	1	9299	6	NULL	NULL	0	NULL	calcium ion	NULL		bind	NULL				ADAM33	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_25_11_2388_s_67	16688218	A calcium ion and a water molecule bound to ADAM33 are represented as green and red  spheres, respectively.	bind
32655	2	9299	6	NULL	NULL	0	NULL	water molecule	NULL		bind	NULL				ADAM33	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_25_11_2388_s_67	16688218	A calcium ion and a water molecule bound to ADAM33 are represented as green and red  spheres, respectively.	bind
40127	2	9300	5	13	NULL	NULL	NULL	statement 1	Process		activates					calcineurin phosphatase	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_3_907_s_28	15657420	A calcium-mediated signaling pathway is involved to activate the calcineurin phosphatase, which binds to the conserved NH2-terminal NFAT homology domain and dephosphorylates NFAT.	bind
40128	4	9300	5	13	NULL	NULL	NULL	calcineurin phosphatase	GP		bind							conserved	NH2-terminal NFAT homology domain		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_3_907_s_28	15657420	A calcium-mediated signaling pathway is involved to activate the calcineurin phosphatase, which binds to the conserved NH2-terminal NFAT homology domain and dephosphorylates NFAT.	bind
40129	3	9300	5	13	NULL	NULL	NULL	statement 2	Process		dephosphorylates					NFAT	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_3_907_s_28	15657420	A calcium-mediated signaling pathway is involved to activate the calcineurin phosphatase, which binds to the conserved NH2-terminal NFAT homology domain and dephosphorylates NFAT.	bind
48102	1	9300	5	13	NULL	NULL	NULL	calcium	Chemical		mediates					signaling pathway	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_3_907_s_28	15657420	A calcium-mediated signaling pathway is involved to activate the calcineurin phosphatase, which binds to the conserved NH2-terminal NFAT homology domain and dephosphorylates NFAT.	bind
32656	1	9300	6	NULL	NULL	0	NULL	calcineurin phosphatase	NULL		bind	NULL					NULL	conserved	NH2-terminal NFAT homology domain		NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_3_907_s_28	15657420	A calcium-mediated signaling pathway is involved to activate the calcineurin phosphatase, which binds to the conserved NH2-terminal NFAT homology domain and dephosphorylates NFAT.	bind
32657	2	9300	6	NULL	NULL	0	NULL	calcineurin phosphatase	NULL		dephosphorylates	NULL				NFAT	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_3_907_s_28	15657420	A calcium-mediated signaling pathway is involved to activate the calcineurin phosphatase, which binds to the conserved NH2-terminal NFAT homology domain and dephosphorylates NFAT.	bind
32658	4	9300	6	10	NULL	0	NULL	statement 3	NULL		is involved in	NULL				calcineurin phosphatase	NULL	activation of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_3_907_s_28	15657420	A calcium-mediated signaling pathway is involved to activate the calcineurin phosphatase, which binds to the conserved NH2-terminal NFAT homology domain and dephosphorylates NFAT.	bind
48103	3	9300	6	10	NULL	0	NULL	calcium	NULL		mediates	NULL				signaling pathway	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_3_907_s_28	15657420	A calcium-mediated signaling pathway is involved to activate the calcineurin phosphatase, which binds to the conserved NH2-terminal NFAT homology domain and dephosphorylates NFAT.	bind
40130	1	9301	5	13	NULL	NULL	NULL	RyR	GP		increase			calmodulin binding domain		spontaneous Ca2+ sparks	Process	activation of			NULL	frog skeletal muscle	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_12_11713_s_1	15640144	A calmodulin binding domain of RyR increases activation of spontaneous Ca2+ sparks in frog skeletal muscle.	bind
32659	1	9301	6	NULL	NULL	0	NULL	RyR	NULL		increases	NULL		calmodulin binding domain		Ca2+ sparks	NULL	activation of 			NULL	frog skeletal muscle	0	NULL	NULL	NULL	gw70_jbiolchem_280_12_11713_s_1	15640144	A calmodulin binding domain of RyR increases activation of spontaneous Ca2+ sparks in frog skeletal muscle.	bind
40131	2	9302	5	13	NULL	NULL	NULL	statement 1	GP		is important for					Ca2+-dependent inactivation	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_477_3_161_s_11	10908714	A calmodulin binding IQ region (1624-1635) within the K-motif has been shown to be important for Ca2+-dependent inactivation [  14,   15 and   16].	bind
48104	1	9302	5	10	NULL	0	NULL		NULL		is located within	NULL		calmodulin binding IQ region (1624-1635)			NULL		K-motif		NULL		0	NULL	NULL	NULL	gw60_febslett_477_3_161_s_11	10908714	A calmodulin binding IQ region (1624-1635) within the K-motif has been shown to be important for Ca2+-dependent inactivation [  14,   15 and   16].	bind
32660	1	9302	6	NULL	NULL	0	NULL		NULL		is located within	NULL		calmodulin binding IQ region (1624-1635)			NULL		K-motif		NULL		0	NULL	NULL	NULL	gw60_febslett_477_3_161_s_11	10908714	A calmodulin binding IQ region (1624-1635) within the K-motif has been shown to be important for Ca2+-dependent inactivation [  14,   15 and   16].	bind
32661	2	9302	6	10	NULL	0	NULL	statement 1			is important for					Ca2+-dependent inactivation					NULL		NULL	NULL	NULL	NULL	gw60_febslett_477_3_161_s_11	10908714	A calmodulin binding IQ region (1624-1635) within the K-motif has been shown to be important for Ca2+-dependent inactivation [  14,   15 and   16].	bind
40132	1	9304	5	13	NULL	NULL	NULL	NE-dlg/SAP102	GP		forms			calmodulin-binding region					basic amphiphilic alpha-helix		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_9_5782_s_35	10026200	A calmodulin-binding region of NE-dlg/SAP102 is predicted to form a basic amphiphilic alpha-helix, which was reported as a calmodulin-binding structure.	bind
40133	2	9304	5	13	NULL	NULL	NULL	basic amphiphilic alpha-helix	GP		is a type of					calmodulin-binding structure	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_9_5782_s_35	10026200	A calmodulin-binding region of NE-dlg/SAP102 is predicted to form a basic amphiphilic alpha-helix, which was reported as a calmodulin-binding structure.	bind
48105	1	9304	6	10	NULL	0	NULL	NE-dlg/SAP102	NULL		forms	NULL		calmodulin-binding region			NULL		basic amphiphilic alpha-helix		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5782_s_35	10026200	A calmodulin-binding region of NE-dlg/SAP102 is predicted to form a basic amphiphilic alpha-helix, which was reported as a calmodulin-binding structure.	bind
48106	2	9304	6	10	NULL	0	NULL	basic amphiphilic alpha-helix	NULL		is a type of	NULL				calmodulin-binding structure	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5782_s_35	10026200	A calmodulin-binding region of NE-dlg/SAP102 is predicted to form a basic amphiphilic alpha-helix, which was reported as a calmodulin-binding structure.	bind
40134	1	9305	5	13	NULL	NULL	NULL	calponin	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20400_s_7	7657614	A calponin peptide (calponin  Phe  -Arg  ), which inhibits the binding of  calponin to actin, blocks the action of calponin and enhances the  contraction induced by submaximal Ca  in permeabilized  vascular smooth muscle.	bind
40135	2	9305	5	13	NULL	NULL	NULL	calponin peptide	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20400_s_7	7657614	A calponin peptide (calponin  Phe  -Arg  ), which inhibits the binding of  calponin to actin, blocks the action of calponin and enhances the  contraction induced by submaximal Ca  in permeabilized  vascular smooth muscle.	bind
40136	3	9305	5	13	NULL	NULL	NULL	calponin peptide	GP		is					calponin Phe -Arg	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20400_s_7	7657614	A calponin peptide (calponin  Phe  -Arg  ), which inhibits the binding of  calponin to actin, blocks the action of calponin and enhances the  contraction induced by submaximal Ca  in permeabilized  vascular smooth muscle.	bind
40137	4	9305	5	13	NULL	NULL	NULL	calponin peptide	GP		block					calponin	GP	action of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20400_s_7	7657614	A calponin peptide (calponin  Phe  -Arg  ), which inhibits the binding of  calponin to actin, blocks the action of calponin and enhances the  contraction induced by submaximal Ca  in permeabilized  vascular smooth muscle.	bind
40138	5	9305	5	13	NULL	NULL	NULL	Ca	Chemical	submaximal	induce					contraction	Process				NULL	permeabilized vascular smooth muscle	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20400_s_7	7657614	A calponin peptide (calponin  Phe  -Arg  ), which inhibits the binding of  calponin to actin, blocks the action of calponin and enhances the  contraction induced by submaximal Ca  in permeabilized  vascular smooth muscle.	bind
40139	6	9305	5	13	NULL	NULL	NULL	calponin peptide	GP		enhance					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20400_s_7	7657614	A calponin peptide (calponin  Phe  -Arg  ), which inhibits the binding of  calponin to actin, blocks the action of calponin and enhances the  contraction induced by submaximal Ca  in permeabilized  vascular smooth muscle.	bind
32707	1	9305	6	NULL	NULL	0	NULL	calponin	NULL		bind	NULL				actin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20400_s_7	7657614	A calponin peptide (calponin  Phe  -Arg  ), which inhibits the binding of  calponin to actin, blocks the action of calponin and enhances the  contraction induced by submaximal Ca  in permeabilized  vascular smooth muscle.	bind
32708	2	9305	6	NULL	NULL	0	NULL	calponin peptide	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20400_s_7	7657614	A calponin peptide (calponin  Phe  -Arg  ), which inhibits the binding of  calponin to actin, blocks the action of calponin and enhances the  contraction induced by submaximal Ca  in permeabilized  vascular smooth muscle.	bind
32709	3	9305	6	NULL	NULL	0	NULL	calponin peptide	NULL		is	NULL				calponin Phe -Arg	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20400_s_7	7657614	A calponin peptide (calponin  Phe  -Arg  ), which inhibits the binding of  calponin to actin, blocks the action of calponin and enhances the  contraction induced by submaximal Ca  in permeabilized  vascular smooth muscle.	bind
32710	4	9305	6	NULL	NULL	0	NULL	calponin peptide	NULL		blocks 	NULL				calponin	NULL	action of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20400_s_7	7657614	A calponin peptide (calponin  Phe  -Arg  ), which inhibits the binding of  calponin to actin, blocks the action of calponin and enhances the  contraction induced by submaximal Ca  in permeabilized  vascular smooth muscle.	bind
32711	5	9305	6	NULL	NULL	0	NULL	Ca	NULL	submaximal	induces	NULL				contraction	NULL				NULL	permeabilized vascular smooth muscle	0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20400_s_7	7657614	A calponin peptide (calponin  Phe  -Arg  ), which inhibits the binding of  calponin to actin, blocks the action of calponin and enhances the  contraction induced by submaximal Ca  in permeabilized  vascular smooth muscle.	bind
32712	6	9305	6	NULL	NULL	0	NULL	calponin peptide	NULL		enhances	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20400_s_7	7657614	A calponin peptide (calponin  Phe  -Arg  ), which inhibits the binding of  calponin to actin, blocks the action of calponin and enhances the  contraction induced by submaximal Ca  in permeabilized  vascular smooth muscle.	bind
40140	1	9306	5	13	NULL	NULL	NULL	CaMKK	GP	pig brain	phosphorylate					AMPK	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_32_29060_s_87	15980064	A CaMKK preparation from pig brain (isolated prior to the recognition that there were two isoforms of the enzyme) has previously been shown to phosphorylate and activate AMPK  in vitro; this phosphorylation is enhanced by the binding of AMP to the AMPK heterotrimer ( ).	bind
40141	2	9306	5	13	NULL	NULL	NULL	statement 1	Process		activates					AMPK	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_32_29060_s_87	15980064	A CaMKK preparation from pig brain (isolated prior to the recognition that there were two isoforms of the enzyme) has previously been shown to phosphorylate and activate AMPK  in vitro; this phosphorylation is enhanced by the binding of AMP to the AMPK heterotrimer ( ).	bind
40142	3	9306	5	13	NULL	NULL	NULL	AMP	Chemical		bind					AMPK heterotrimer	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_32_29060_s_87	15980064	A CaMKK preparation from pig brain (isolated prior to the recognition that there were two isoforms of the enzyme) has previously been shown to phosphorylate and activate AMPK  in vitro; this phosphorylation is enhanced by the binding of AMP to the AMPK heterotrimer ( ).	bind
40143	4	9306	5	13	NULL	NULL	NULL	statement 3	Process		enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_32_29060_s_87	15980064	A CaMKK preparation from pig brain (isolated prior to the recognition that there were two isoforms of the enzyme) has previously been shown to phosphorylate and activate AMPK  in vitro; this phosphorylation is enhanced by the binding of AMP to the AMPK heterotrimer ( ).	bind
32979	1	9306	6	NULL	NULL	0	NULL	AMP	NULL		bind	NULL				AMPK heterotrimer	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_32_29060_s_87	15980064	A CaMKK preparation from pig brain (isolated prior to the recognition that there were two isoforms of the enzyme) has previously been shown to phosphorylate and activate AMPK  in vitro; this phosphorylation is enhanced by the binding of AMP to the AMPK heterotrimer ( ).	bind
32980	2	9306	6	NULL	NULL	0	NULL	CaMKK	NULL	pig brain	phosphorylate	NULL				AMPK	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw70_jbiolchem_280_32_29060_s_87	15980064	A CaMKK preparation from pig brain (isolated prior to the recognition that there were two isoforms of the enzyme) has previously been shown to phosphorylate and activate AMPK  in vitro; this phosphorylation is enhanced by the binding of AMP to the AMPK heterotrimer ( ).	bind
32981	3	9306	6	NULL	NULL	0	NULL	CaMKK	NULL	pig brain	activate	NULL				AMPK	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw70_jbiolchem_280_32_29060_s_87	15980064	A CaMKK preparation from pig brain (isolated prior to the recognition that there were two isoforms of the enzyme) has previously been shown to phosphorylate and activate AMPK  in vitro; this phosphorylation is enhanced by the binding of AMP to the AMPK heterotrimer ( ).	bind
32982	4	9306	6	NULL	NULL	0	NULL	statement 1	NULL		enhances	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_32_29060_s_87	15980064	A CaMKK preparation from pig brain (isolated prior to the recognition that there were two isoforms of the enzyme) has previously been shown to phosphorylate and activate AMPK  in vitro; this phosphorylation is enhanced by the binding of AMP to the AMPK heterotrimer ( ).	bind
40144	1	9307	5	13	NULL	NULL	NULL				is present 				cAMP response element	immediate early genes	GP	upstream of 			NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_111_1_1_s_112	12654499	A cAMP response element can  be found upstream of the immediate early genes [  21], and this DNA region is bound by the phosphorylated form of CREB [ 6.	bind
40145	2	9307	5	13	NULL	NULL	NULL	CREB	GP	phosphorylated	bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_111_1_1_s_112	12654499	A cAMP response element can  be found upstream of the immediate early genes [  21], and this DNA region is bound by the phosphorylated form of CREB [ 6.	bind
32983	2	9307	6	10	NULL	0	NULL	statement 1	NULL		bind	NULL				CREB	NULL	phosphorylated form of			NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_111_1_1_s_112	12654499	A cAMP response element can  be found upstream of the immediate early genes [  21], and this DNA region is bound by the phosphorylated form of CREB [ 6.	bind
48107	1	9307	6	10	NULL	0	NULL		NULL		is present	NULL			cAMP response element	immediate early genes	NULL	upstream of			NULL		NULL	NULL	NULL	NULL	gw70_brainresmolbrainres_111_1_1_s_112	12654499	A cAMP response element can  be found upstream of the immediate early genes [  21], and this DNA region is bound by the phosphorylated form of CREB [ 6.	bind
40146	1	9309	5	13	NULL	NULL	NULL				undergoes			subunit IV		phosphorylation	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_466_1_130_s_74	10648827	A cAMP-independent phosphorylation of subunit IV, to which ATP binds and induces the allosteric ATP-inhibition [ 4, has been described by Steenaart and Shore [ 11].	bind
40147	2	9309	5	13	NULL	NULL	NULL	statement 1	Process		is independent of					cAMP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_466_1_130_s_74	10648827	A cAMP-independent phosphorylation of subunit IV, to which ATP binds and induces the allosteric ATP-inhibition [ 4, has been described by Steenaart and Shore [ 11].	bind
40148	3	9309	5	13	NULL	NULL	NULL	ATP	Chemical		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_466_1_130_s_74	10648827	A cAMP-independent phosphorylation of subunit IV, to which ATP binds and induces the allosteric ATP-inhibition [ 4, has been described by Steenaart and Shore [ 11].	bind
40149	4	9309	5	13	NULL	NULL	NULL	statement 3	Process		induce					ATP	Chemical	allosteric inhibition of			NULL		NULL	NULL	NULL	NULL	gw60_febslett_466_1_130_s_74	10648827	A cAMP-independent phosphorylation of subunit IV, to which ATP binds and induces the allosteric ATP-inhibition [ 4, has been described by Steenaart and Shore [ 11].	bind
32984	1	9309	6	10	NULL	0	NULL			phosphorylated	bind			subunit IV		ATP					NULL		NULL	NULL	NULL	NULL	gw60_febslett_466_1_130_s_74	10648827	A cAMP-independent phosphorylation of subunit IV, to which ATP binds and induces the allosteric ATP-inhibition [ 4, has been described by Steenaart and Shore [ 11].	bind
32985	2	9309	6	10	NULL	0	NULL				induces			subunit IV		ATP		allosteric;; inhibition of 			NULL		NULL	NULL	NULL	NULL	gw60_febslett_466_1_130_s_74	10648827	A cAMP-independent phosphorylation of subunit IV, to which ATP binds and induces the allosteric ATP-inhibition [ 4, has been described by Steenaart and Shore [ 11].	bind
32986	3	9309	6	10	NULL	0	NULL			phosphorylation of	is independent of			subunit IV		cAMP					NULL		NULL	NULL	NULL	NULL	gw60_febslett_466_1_130_s_74	10648827	A cAMP-independent phosphorylation of subunit IV, to which ATP binds and induces the allosteric ATP-inhibition [ 4, has been described by Steenaart and Shore [ 11].	bind
40150	1	9310	5	13	NULL	NULL	NULL	ABL kinase inhibitor	GP		bind								SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_32_19585_s_19	8702653	A candidate ABL kinase inhibitor that binds to the SH3 domain has been purified, and this protein exhibits GTPase-activating protein homology, implying that ABL may interact with the ras related proteins ( 19).	bind
40151	2	9310	5	13	NULL	NULL	NULL	ABL kinase inhibitor	GP		is homologous to					GTPase-activating protein 	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_32_19585_s_19	8702653	A candidate ABL kinase inhibitor that binds to the SH3 domain has been purified, and this protein exhibits GTPase-activating protein homology, implying that ABL may interact with the ras related proteins ( 19).	bind
40152	3	9310	5	13	NULL	NULL	NULL	ABL	GP		interact with		may			ras related proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_32_19585_s_19	8702653	A candidate ABL kinase inhibitor that binds to the SH3 domain has been purified, and this protein exhibits GTPase-activating protein homology, implying that ABL may interact with the ras related proteins ( 19).	bind
40153	4	9310	5	13	NULL	NULL	NULL	statement 2	Process		implies					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_32_19585_s_19	8702653	A candidate ABL kinase inhibitor that binds to the SH3 domain has been purified, and this protein exhibits GTPase-activating protein homology, implying that ABL may interact with the ras related proteins ( 19).	bind
32987	1	9310	6	NULL	NULL	0	NULL	ABL kinase inhibitor	NULL		bind	NULL					NULL		SH3 domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_32_19585_s_19	8702653	A candidate ABL kinase inhibitor that binds to the SH3 domain has been purified, and this protein exhibits GTPase-activating protein homology, implying that ABL may interact with the ras related proteins ( 19).	bind
32988	2	9310	6	10	NULL	0	NULL	ABL kinase inhibitor	NULL		is homologous to	NULL				GTPase-activating protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_32_19585_s_19	8702653	A candidate ABL kinase inhibitor that binds to the SH3 domain has been purified, and this protein exhibits GTPase-activating protein homology, implying that ABL may interact with the ras related proteins ( 19).	bind
32989	3	9310	6	NULL	NULL	0	NULL	ABL	NULL		interacts with	NULL	may			ras related proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_32_19585_s_19	8702653	A candidate ABL kinase inhibitor that binds to the SH3 domain has been purified, and this protein exhibits GTPase-activating protein homology, implying that ABL may interact with the ras related proteins ( 19).	bind
32990	4	9310	6	NULL	NULL	0	NULL	statement 2	NULL		implies	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_32_19585_s_19	8702653	A candidate ABL kinase inhibitor that binds to the SH3 domain has been purified, and this protein exhibits GTPase-activating protein homology, implying that ABL may interact with the ras related proteins ( 19).	bind
40154	1	9311	5	13	NULL	NULL	NULL	 anchoring/targeting protein	GP		bind					PKC3	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_2_1130_s_15	9422779	A candidate anchoring/targeting protein, which binds PKC3  in vitro, has been identified.	bind
32991	1	9311	6	NULL	NULL	0	NULL	anchoring/targeting protein	NULL		bind	NULL				PKC3	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_273_2_1130_s_15	9422779	A candidate anchoring/targeting protein, which binds PKC3  in vitro, has been identified.	bind
40385	1	9312	5	13	NULL	NULL	NULL	mammalian homolog to Upf1p	GP	S. cerevisiae	is involved in					decay	Process	nonsense-mediated			NULL	S. cerevisiae	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5272_s_288	9710612	A candidate for such a factor could be the mammalian homolog to  S. cerevisiae Upf1p, a factor involved in nonsense-mediated decay in  S. cerevisiae that is characterized by RNA binding and helicase activities ( 44).	bind
40386	2	9312	5	13	NULL	NULL	NULL	mammalian homolog to Upf1p	GP	S. cerevisiae	bind					RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5272_s_288	9710612	A candidate for such a factor could be the mammalian homolog to  S. cerevisiae Upf1p, a factor involved in nonsense-mediated decay in  S. cerevisiae that is characterized by RNA binding and helicase activities ( 44).	bind
40387	3	9312	5	13	NULL	NULL	NULL	statement 1	Process		is characterized by					helicase	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5272_s_288	9710612	A candidate for such a factor could be the mammalian homolog to  S. cerevisiae Upf1p, a factor involved in nonsense-mediated decay in  S. cerevisiae that is characterized by RNA binding and helicase activities ( 44).	bind
48108	4	9312	5	13	NULL	NULL	NULL	statement 1	Process		is characterized by					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5272_s_288	9710612	A candidate for such a factor could be the mammalian homolog to  S. cerevisiae Upf1p, a factor involved in nonsense-mediated decay in  S. cerevisiae that is characterized by RNA binding and helicase activities ( 44).	bind
33882	1	9312	6	10	NULL	0	NULL	mammalian homolog to Upf1p		 S. cerevisiae	is involved in					 decay		nonsense-mediated			NULL	S.cerevisiae	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5272_s_288	9710612	A candidate for such a factor could be the mammalian homolog to  S. cerevisiae Upf1p, a factor involved in nonsense-mediated decay in  S. cerevisiae that is characterized by RNA binding and helicase activities ( 44).	bind
33883	2	9312	6	10	NULL	0	NULL	mammalian homolog to Upf1p	NULL	 S. cerevisiae	bind	NULL				RNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5272_s_288	9710612	A candidate for such a factor could be the mammalian homolog to  S. cerevisiae Upf1p, a factor involved in nonsense-mediated decay in  S. cerevisiae that is characterized by RNA binding and helicase activities ( 44).	bind
33885	4	9312	6	NULL	NULL	0	NULL	statement 1	NULL		is characterized by	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_9_5272_s_288	9710612	A candidate for such a factor could be the mammalian homolog to  S. cerevisiae Upf1p, a factor involved in nonsense-mediated decay in  S. cerevisiae that is characterized by RNA binding and helicase activities ( 44).	bind
33886	3	9312	6	10	NULL	0	NULL	statement 1			is characterized by					helicase		activity of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5272_s_288	9710612	A candidate for such a factor could be the mammalian homolog to  S. cerevisiae Upf1p, a factor involved in nonsense-mediated decay in  S. cerevisiae that is characterized by RNA binding and helicase activities ( 44).	bind
40155	1	9313	5	13	NULL	NULL	NULL	heparin	Chemical		bind					P4n	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_21_18421_s_341	11882649	A candidate for such a site is P4n-(110-128), and preliminary observations in our laboratory, not presented here, indicate that heparin binding of P4n is abrogated by Cu(II).	bind
40156	2	9313	5	13	NULL	NULL	NULL	Cu(II)	Chemical		abrogates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_21_18421_s_341	11882649	A candidate for such a site is P4n-(110-128), and preliminary observations in our laboratory, not presented here, indicate that heparin binding of P4n is abrogated by Cu(II).	bind
32992	1	9313	6	NULL	NULL	0	NULL	heparin	NULL		bind	NULL				P4n	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_21_18421_s_341	11882649	A candidate for such a site is P4n-(110-128), and preliminary observations in our laboratory, not presented here, indicate that heparin binding of P4n is abrogated by Cu(II).	bind
32993	2	9313	6	NULL	NULL	0	NULL	Cu(II)	NULL		abrogates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_21_18421_s_341	11882649	A candidate for such a site is P4n-(110-128), and preliminary observations in our laboratory, not presented here, indicate that heparin binding of P4n is abrogated by Cu(II).	bind
40157	1	9314	5	13	NULL	NULL	NULL	beta3-endonexin	GP		contains								Tyr residue		NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_6_1651_s_234	10845885	A candidate is beta3-endonexin, which contains a Tyr residue and in Chinese hamster ovary cells binds to the beta3 cytoplasmic tail, thereby increasing ligand binding to alphaIIbbeta3.	bind
40158	2	9314	5	13	NULL	NULL	NULL	statement 1	GP		bind					beta3	GP		cytoplasmic tail		NULL	Chinese hamster ovary cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_6_1651_s_234	10845885	A candidate is beta3-endonexin, which contains a Tyr residue and in Chinese hamster ovary cells binds to the beta3 cytoplasmic tail, thereby increasing ligand binding to alphaIIbbeta3.	bind
40159	3	9314	5	13	NULL	NULL	NULL	ligand	GP		bind					alphaIIbbeta3	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_6_1651_s_234	10845885	A candidate is beta3-endonexin, which contains a Tyr residue and in Chinese hamster ovary cells binds to the beta3 cytoplasmic tail, thereby increasing ligand binding to alphaIIbbeta3.	bind
40160	4	9314	5	13	NULL	NULL	NULL	statement 2	Process		increase					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_6_1651_s_234	10845885	A candidate is beta3-endonexin, which contains a Tyr residue and in Chinese hamster ovary cells binds to the beta3 cytoplasmic tail, thereby increasing ligand binding to alphaIIbbeta3.	bind
32994	1	9314	6	10	NULL	0	NULL	beta3-endonexin	NULL		contains 	NULL				Tyr residue	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_6_1651_s_234	10845885	A candidate is beta3-endonexin, which contains a Tyr residue and in Chinese hamster ovary cells binds to the beta3 cytoplasmic tail, thereby increasing ligand binding to alphaIIbbeta3.	bind
32995	2	9314	6	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL				beta3	NULL		cytoplasmic tail		NULL	Chinese hamster ovary cells	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_6_1651_s_234	10845885	A candidate is beta3-endonexin, which contains a Tyr residue and in Chinese hamster ovary cells binds to the beta3 cytoplasmic tail, thereby increasing ligand binding to alphaIIbbeta3.	bind
33004	3	9314	6	NULL	NULL	0	NULL	alphaIIbbeta3	NULL		bind	NULL				ligand	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_6_1651_s_234	10845885	A candidate is beta3-endonexin, which contains a Tyr residue and in Chinese hamster ovary cells binds to the beta3 cytoplasmic tail, thereby increasing ligand binding to alphaIIbbeta3.	bind
33005	4	9314	6	NULL	NULL	0	NULL	statement 2	NULL		increases	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_6_1651_s_234	10845885	A candidate is beta3-endonexin, which contains a Tyr residue and in Chinese hamster ovary cells binds to the beta3 cytoplasmic tail, thereby increasing ligand binding to alphaIIbbeta3.	bind
40161	1	9315	5	13	NULL	NULL	NULL	KIF-4	GP		is a type of					kinesin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_3_393_s_43	12427864	A candidate motor for this transport is KIF-4, a kinesin that can bind to the matrix protein of HIV and SIV ( Tang et al., 1999).	bind
40162	2	9315	5	13	NULL	NULL	NULL	KIF-4	GP		bind					matrix protein	GP	HIV			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_3_393_s_43	12427864	A candidate motor for this transport is KIF-4, a kinesin that can bind to the matrix protein of HIV and SIV ( Tang et al., 1999).	bind
40163	3	9315	5	13	NULL	NULL	NULL	KIF-4	GP		bind					matrix protein	GP	SIV			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_159_3_393_s_43	12427864	A candidate motor for this transport is KIF-4, a kinesin that can bind to the matrix protein of HIV and SIV ( Tang et al., 1999).	bind
33007	1	9315	6	NULL	NULL	0	NULL	KIF-4	NULL		is a type of	NULL				kinesin	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_159_3_393_s_43	12427864	A candidate motor for this transport is KIF-4, a kinesin that can bind to the matrix protein of HIV and SIV ( Tang et al., 1999).	bind
33008	2	9315	6	NULL	NULL	0	NULL	KIF-4	NULL		bind	NULL				matrix protein	NULL	HIV			NULL		0	NULL	NULL	NULL	gw60_cellbiol_159_3_393_s_43	12427864	A candidate motor for this transport is KIF-4, a kinesin that can bind to the matrix protein of HIV and SIV ( Tang et al., 1999).	bind
33010	3	9315	6	NULL	NULL	0	NULL	KIF-4	NULL		bind	NULL				matrix protein	NULL	SIV			NULL		0	NULL	NULL	NULL	gw60_cellbiol_159_3_393_s_43	12427864	A candidate motor for this transport is KIF-4, a kinesin that can bind to the matrix protein of HIV and SIV ( Tang et al., 1999).	bind
40164	2	9316	5	13	NULL	NULL	NULL	AP-2	GP		is a candidate of					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1635_2_104_s_353	14729073	A candidate of the PMA-responsive transcription factor that binds AP-2 site is, of  course, AP-2 [  42 and   43].	bind
40165	3	9316	5	13	NULL	NULL	NULL	AP-2	GP		bind									AP-2 site	NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1635_2_104_s_353	14729073	A candidate of the PMA-responsive transcription factor that binds AP-2 site is, of  course, AP-2 [  42 and   43].	bind
48109	1	9316	5	13	NULL	NULL	NULL	transcription factor	GP		respond to					PMA	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1635_2_104_s_353	14729073	A candidate of the PMA-responsive transcription factor that binds AP-2 site is, of  course, AP-2 [  42 and   43].	bind
33011	2	9316	6	10	NULL	0	NULL	AP-2			is a candidate of					statement 1					NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1635_2_104_s_353	14729073	A candidate of the PMA-responsive transcription factor that binds AP-2 site is, of  course, AP-2 [  42 and   43].	bind
33012	3	9316	6	10	NULL	0	NULL	AP-2	NULL		bind	NULL					NULL			AP-2 site	NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1635_2_104_s_353	14729073	A candidate of the PMA-responsive transcription factor that binds AP-2 site is, of  course, AP-2 [  42 and   43].	bind
48110	1	9316	6	10	NULL	0	NULL	transcription factor	NULL		respond to	NULL				PMA	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1635_2_104_s_353	14729073	A candidate of the PMA-responsive transcription factor that binds AP-2 site is, of  course, AP-2 [  42 and   43].	bind
40166	1	9317	5	13	NULL	NULL	NULL	 calmodulin	GP		activates					PI3K	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_7591_s_235	12488453	A candidate target protein for activation of PI3K by calmodulin is Ras because it has been reported that calmodulin can bind directly to Ras and modulate its downstream signaling ( 52).	bind
40167	2	9317	5	13	NULL	NULL	NULL	calmodulin	GP		bind		directly			Ras	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_7591_s_235	12488453	A candidate target protein for activation of PI3K by calmodulin is Ras because it has been reported that calmodulin can bind directly to Ras and modulate its downstream signaling ( 52).	bind
40168	3	9317	5	13	NULL	NULL	NULL	statement 2	Process		modulates					Ras	GP	downstream signaling of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_7591_s_235	12488453	A candidate target protein for activation of PI3K by calmodulin is Ras because it has been reported that calmodulin can bind directly to Ras and modulate its downstream signaling ( 52).	bind
33013	1	9317	6	NULL	NULL	0	NULL	Calmodulin	NULL		bind	NULL	directly			Ras	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_9_7591_s_235	12488453	A candidate target protein for activation of PI3K by calmodulin is Ras because it has been reported that calmodulin can bind directly to Ras and modulate its downstream signaling ( 52).	bind
33015	2	9317	6	NULL	NULL	0	NULL	Calmodulin	NULL		activates	NULL				PI3K	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_9_7591_s_235	12488453	A candidate target protein for activation of PI3K by calmodulin is Ras because it has been reported that calmodulin can bind directly to Ras and modulate its downstream signaling ( 52).	bind
33016	3	9317	6	NULL	NULL	0	NULL	Calmodulin	NULL		modulates	NULL				Ras	NULL	downstream signaling of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_9_7591_s_235	12488453	A candidate target protein for activation of PI3K by calmodulin is Ras because it has been reported that calmodulin can bind directly to Ras and modulate its downstream signaling ( 52).	bind
40169	1	9318	5	13	NULL	NULL	NULL	Crb	GP		is a type of					 transmembrane protein	GP	epithelium			NULL		NULL	NULL	NULL	NULL	gw70_mechdev_120_11_1297_s_45	14623439	A candidate transmembrane protein in the epithelium is Crb, which  binds directly to the MAGUK protein Sdt ([ Bachmann et al., 2001,  Hong et al., 2001 and   Roh et al., 2002]).	bind
40170	2	9318	5	13	NULL	NULL	NULL	Crb	GP		bind		directly			Sdt	GP				NULL		NULL	NULL	NULL	NULL	gw70_mechdev_120_11_1297_s_45	14623439	A candidate transmembrane protein in the epithelium is Crb, which  binds directly to the MAGUK protein Sdt ([ Bachmann et al., 2001,  Hong et al., 2001 and   Roh et al., 2002]).	bind
40171	3	9318	5	13	NULL	NULL	NULL	Sdt	GP		is a type of					MAGUK	GP				NULL		NULL	NULL	NULL	NULL	gw70_mechdev_120_11_1297_s_45	14623439	A candidate transmembrane protein in the epithelium is Crb, which  binds directly to the MAGUK protein Sdt ([ Bachmann et al., 2001,  Hong et al., 2001 and   Roh et al., 2002]).	bind
33017	1	9318	6	NULL	NULL	0	NULL	Crb	NULL		bind	NULL	directly			Sdt	NULL				NULL		NULL	NULL	NULL	NULL	gw70_mechdev_120_11_1297_s_45	14623439	A candidate transmembrane protein in the epithelium is Crb, which  binds directly to the MAGUK protein Sdt ([ Bachmann et al., 2001,  Hong et al., 2001 and   Roh et al., 2002]).	bind
33018	2	9318	6	10	NULL	0	NULL	Crb	NULL		is a type of	NULL				transmembrane protein	NULL	epithelium			NULL		NULL	NULL	NULL	NULL	gw70_mechdev_120_11_1297_s_45	14623439	A candidate transmembrane protein in the epithelium is Crb, which  binds directly to the MAGUK protein Sdt ([ Bachmann et al., 2001,  Hong et al., 2001 and   Roh et al., 2002]).	bind
33021	3	9318	6	NULL	NULL	0	NULL	Sdt	NULL		is a type of	NULL				MAGUK protein	NULL				NULL		0	NULL	NULL	NULL	gw70_mechdev_120_11_1297_s_45	14623439	A candidate transmembrane protein in the epithelium is Crb, which  binds directly to the MAGUK protein Sdt ([ Bachmann et al., 2001,  Hong et al., 2001 and   Roh et al., 2002]).	bind
40186	1	9319	5	13	NULL	NULL	NULL				bind				Meg1 repeat	CTCF	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_5_1398_s_120	12595547	A canonical CTCF-binding sequence from chicken beta- globin (FII) specifically competed CTCF binding to the  Meg1 repeat (lane indicated by competitor F), although the recognition sequences for the SP1 and AP1 transcription factors did not interfere with CTCF binding (lanes indicated by competitors S and A).	bind
40187	2	9319	5	13	NULL	NULL	NULL	beta- globin (FII)	GP	chicken	bind				canonical CTCF-binding sequence					Meg1 repeat	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_5_1398_s_120	12595547	A canonical CTCF-binding sequence from chicken beta- globin (FII) specifically competed CTCF binding to the  Meg1 repeat (lane indicated by competitor F), although the recognition sequences for the SP1 and AP1 transcription factors did not interfere with CTCF binding (lanes indicated by competitors S and A).	bind
40188	3	9319	5	13	NULL	NULL	NULL	statement 2	Process		competes with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_5_1398_s_120	12595547	A canonical CTCF-binding sequence from chicken beta- globin (FII) specifically competed CTCF binding to the  Meg1 repeat (lane indicated by competitor F), although the recognition sequences for the SP1 and AP1 transcription factors did not interfere with CTCF binding (lanes indicated by competitors S and A).	bind
40189	4	9319	5	13	NULL	NULL	NULL	SP1	GP		does not interfere with				recognition sequences	CTCF	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_5_1398_s_120	12595547	A canonical CTCF-binding sequence from chicken beta- globin (FII) specifically competed CTCF binding to the  Meg1 repeat (lane indicated by competitor F), although the recognition sequences for the SP1 and AP1 transcription factors did not interfere with CTCF binding (lanes indicated by competitors S and A).	bind
40190	5	9319	5	13	NULL	NULL	NULL	AP1	GP		does not interfere with				recognition sequences	CTCF	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_5_1398_s_120	12595547	A canonical CTCF-binding sequence from chicken beta- globin (FII) specifically competed CTCF binding to the  Meg1 repeat (lane indicated by competitor F), although the recognition sequences for the SP1 and AP1 transcription factors did not interfere with CTCF binding (lanes indicated by competitors S and A).	bind
40191	6	9319	5	13	NULL	NULL	NULL	AP1	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_5_1398_s_120	12595547	A canonical CTCF-binding sequence from chicken beta- globin (FII) specifically competed CTCF binding to the  Meg1 repeat (lane indicated by competitor F), although the recognition sequences for the SP1 and AP1 transcription factors did not interfere with CTCF binding (lanes indicated by competitors S and A).	bind
40192	7	9319	5	13	NULL	NULL	NULL	SP1	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_5_1398_s_120	12595547	A canonical CTCF-binding sequence from chicken beta- globin (FII) specifically competed CTCF binding to the  Meg1 repeat (lane indicated by competitor F), although the recognition sequences for the SP1 and AP1 transcription factors did not interfere with CTCF binding (lanes indicated by competitors S and A).	bind
33087	1	9319	6	NULL	NULL	0	NULL	CTCF	NULL		bind	NULL					NULL			Meg1 repeat	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_5_1398_s_120	12595547	A canonical CTCF-binding sequence from chicken beta- globin (FII) specifically competed CTCF binding to the  Meg1 repeat (lane indicated by competitor F), although the recognition sequences for the SP1 and AP1 transcription factors did not interfere with CTCF binding (lanes indicated by competitors S and A).	bind
33887	2	9319	6	NULL	NULL	0	NULL	beta- globin (FII)	NULL	chicken	bind	NULL			CTCF-binding sequence		NULL			Meg1 repeat	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_5_1398_s_120	12595547	A canonical CTCF-binding sequence from chicken beta- globin (FII) specifically competed CTCF binding to the  Meg1 repeat (lane indicated by competitor F), although the recognition sequences for the SP1 and AP1 transcription factors did not interfere with CTCF binding (lanes indicated by competitors S and A).	bind
33888	3	9319	6	NULL	NULL	0	NULL	statement 1	NULL		competes	NULL	specifically			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_5_1398_s_120	12595547	A canonical CTCF-binding sequence from chicken beta- globin (FII) specifically competed CTCF binding to the  Meg1 repeat (lane indicated by competitor F), although the recognition sequences for the SP1 and AP1 transcription factors did not interfere with CTCF binding (lanes indicated by competitors S and A).	bind
48111	4	9319	6	10	NULL	0	NULL	SP1	NULL		does not interfere with	NULL			recognition sequences	CTCF	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_5_1398_s_120	12595547	A canonical CTCF-binding sequence from chicken beta- globin (FII) specifically competed CTCF binding to the  Meg1 repeat (lane indicated by competitor F), although the recognition sequences for the SP1 and AP1 transcription factors did not interfere with CTCF binding (lanes indicated by competitors S and A).	bind
48112	5	9319	6	10	NULL	0	NULL	AP1	NULL		does not interfere with	NULL			recognition sequences	CTCF	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_5_1398_s_120	12595547	A canonical CTCF-binding sequence from chicken beta- globin (FII) specifically competed CTCF binding to the  Meg1 repeat (lane indicated by competitor F), although the recognition sequences for the SP1 and AP1 transcription factors did not interfere with CTCF binding (lanes indicated by competitors S and A).	bind
48113	6	9319	6	10	NULL	0	NULL	AP1	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_5_1398_s_120	12595547	A canonical CTCF-binding sequence from chicken beta- globin (FII) specifically competed CTCF binding to the  Meg1 repeat (lane indicated by competitor F), although the recognition sequences for the SP1 and AP1 transcription factors did not interfere with CTCF binding (lanes indicated by competitors S and A).	bind
48114	7	9319	6	10	NULL	0	NULL	SP1	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_5_1398_s_120	12595547	A canonical CTCF-binding sequence from chicken beta- globin (FII) specifically competed CTCF binding to the  Meg1 repeat (lane indicated by competitor F), although the recognition sequences for the SP1 and AP1 transcription factors did not interfere with CTCF binding (lanes indicated by competitors S and A).	bind
40180	1	9320	5	13	NULL	NULL	NULL	Jun	GP		is activated by					EGF	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_10_9634_s_152	14676207	A canonical DEF domain rescues Jun activation by EGF.	bind
40181	2	9320	5	13	NULL	NULL	NULL			canonical	rescues			 DEF domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_10_9634_s_152	14676207	A canonical DEF domain rescues Jun activation by EGF.	bind
33088	1	9320	6	NULL	NULL	0	NULL	EGF	NULL		activates	NULL				Jun	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_10_9634_s_152	14676207	A canonical DEF domain rescues Jun activation by EGF.	bind
33089	2	9320	6	NULL	NULL	0	NULL		NULL	canonical	rescues	NULL		DEF domain		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_10_9634_s_152	14676207	A canonical DEF domain rescues Jun activation by EGF.	bind
40183	1	9321	5	13	NULL	NULL	NULL	Wnt proteins	GP	secreted	bind					Frizzled receptors	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_17_6027_s_248	15837931	A canonical pathway activated by the secreted Wnt proteins binding to the Frizzled receptors has been well characterized ( ,  ).	bind
40184	2	9321	5	13	NULL	NULL	NULL	statement 1	Process		activates					canonical pathway	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_17_6027_s_248	15837931	A canonical pathway activated by the secreted Wnt proteins binding to the Frizzled receptors has been well characterized ( ,  ).	bind
33113	1	9321	6	NULL	NULL	0	NULL	Wnt proteins	NULL	secreted	bind	NULL				Frizzled receptors	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_17_6027_s_248	15837931	A canonical pathway activated by the secreted Wnt proteins binding to the Frizzled receptors has been well characterized ( ,  ).	bind
58461	2	9321	6	10	NULL	0	NULL	statement 1			activates					canonical pathway					NULL		0	NULL	NULL	NULL	gw70_pnas_102_17_6027_s_248	15837931	A canonical pathway activated by the secreted Wnt proteins binding to the Frizzled receptors has been well characterized ( ,  ).	bind
40185	1	9322	5	13	NULL	NULL	NULL	I-GST	GP		does not bind		directly			ICAM-1 mAb	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_6_3358_s_110	9452454	A capture ELISA assay showed that there is no direct binding of I-GST to any ICAM-1 mAb tested (data not shown).	bind
33115	1	9322	6	NULL	NULL	0	NULL	I-GST	NULL		does not bind	NULL	directly			ICAM-1 mAb	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_6_3358_s_110	9452454	A capture ELISA assay showed that there is no direct binding of I-GST to any ICAM-1 mAb tested (data not shown).	bind
40207	1	9324	5	NULL	NULL	0	NULL		NULL	deletion of	include	NULL		carboxy-terminal (aa 1 to 138)			NULL		putative TPR motifs		NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_20_8938_s_107	15456868	A carboxy-terminal deletion (amino acids 1 to 138) that only includes the three putative TPR motifs bound to Ctf13p but failed to bind to Skp1p.	bind
40209	2	9324	5	13	NULL	NULL	NULL	statement 1	GP		bind					Ctf13p	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_8938_s_107	15456868	A carboxy-terminal deletion (amino acids 1 to 138) that only includes the three putative TPR motifs bound to Ctf13p but failed to bind to Skp1p.	bind
40210	3	9324	5	13	NULL	NULL	NULL	statement 1	GP		does not bind					Skp1p	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_20_8938_s_107	15456868	A carboxy-terminal deletion (amino acids 1 to 138) that only includes the three putative TPR motifs bound to Ctf13p but failed to bind to Skp1p.	bind
33116	1	9324	6	NULL	NULL	0	NULL		NULL	deletion of	includes	NULL		carboxy-terminal (amino acids 1 to 138)			NULL	putative	TPR motifs		NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_20_8938_s_107	15456868	A carboxy-terminal deletion (amino acids 1 to 138) that only includes the three putative TPR motifs bound to Ctf13p but failed to bind to Skp1p.	bind
33117	2	9324	6	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL				Ctf13p	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_20_8938_s_107	15456868	A carboxy-terminal deletion (amino acids 1 to 138) that only includes the three putative TPR motifs bound to Ctf13p but failed to bind to Skp1p.	bind
33118	3	9324	6	NULL	NULL	0	NULL	statement 1	NULL		does not bind	NULL				Skp1p	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_20_8938_s_107	15456868	A carboxy-terminal deletion (amino acids 1 to 138) that only includes the three putative TPR motifs bound to Ctf13p but failed to bind to Skp1p.	bind
40202	1	9325	5	13	NULL	NULL	NULL	p53	GP		bind			carboxy-terminal region		XPB	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_9_1057_s_42	8805363	A carboxy-terminal region of p53 binds to XPB and XPD and this region of p53 inhibits their DNA helicase activities    [7,8,10]  .	bind
40203	2	9325	5	13	NULL	NULL	NULL	p53	GP		bind			carboxy-terminal region		XPD	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_9_1057_s_42	8805363	A carboxy-terminal region of p53 binds to XPB and XPD and this region of p53 inhibits their DNA helicase activities    [7,8,10]  .	bind
40204	5	9325	5	13	NULL	NULL	NULL	p53	GP		inhibit			carboxy-terminal region		statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_9_1057_s_42	8805363	A carboxy-terminal region of p53 binds to XPB and XPD and this region of p53 inhibits their DNA helicase activities    [7,8,10]  .	bind
40205	6	9325	5	13	NULL	NULL	NULL	p53	GP		inhibit			carboxy-terminal region		statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_9_1057_s_42	8805363	A carboxy-terminal region of p53 binds to XPB and XPD and this region of p53 inhibits their DNA helicase activities    [7,8,10]  .	bind
58462	3	9325	5	13	NULL	NULL	NULL	XPB	GP		activates					DNA helicase	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_9_1057_s_42	8805363	A carboxy-terminal region of p53 binds to XPB and XPD and this region of p53 inhibits their DNA helicase activities    [7,8,10]  .	bind
58463	4	9325	5	13	NULL	NULL	NULL	XPD	GP		activates					DNA helicase	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_9_1057_s_42	8805363	A carboxy-terminal region of p53 binds to XPB and XPD and this region of p53 inhibits their DNA helicase activities    [7,8,10]  .	bind
33119	1	9325	6	NULL	NULL	0	NULL	p53	NULL		bind	NULL		carboxy-terminal region		XPB	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_6_9_1057_s_42	8805363	A carboxy-terminal region of p53 binds to XPB and XPD and this region of p53 inhibits their DNA helicase activities    [7,8,10]  .	bind
33120	2	9325	6	NULL	NULL	0	NULL	p53	NULL		bind	NULL		carboxy-terminal region		XPD	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_6_9_1057_s_42	8805363	A carboxy-terminal region of p53 binds to XPB and XPD and this region of p53 inhibits their DNA helicase activities    [7,8,10]  .	bind
33121	3	9325	6	10	NULL	0	NULL	XPB			activates					DNA helicase					NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_9_1057_s_42	8805363	A carboxy-terminal region of p53 binds to XPB and XPD and this region of p53 inhibits their DNA helicase activities    [7,8,10]  .	bind
33122	4	9325	6	10	NULL	0	NULL	XPD			activates					DNA helicase					NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_9_1057_s_42	8805363	A carboxy-terminal region of p53 binds to XPB and XPD and this region of p53 inhibits their DNA helicase activities    [7,8,10]  .	bind
33123	5	9325	6	NULL	NULL	0	NULL	p53	NULL		inhibits	NULL		carboxy-terminal region		statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_6_9_1057_s_42	8805363	A carboxy-terminal region of p53 binds to XPB and XPD and this region of p53 inhibits their DNA helicase activities    [7,8,10]  .	bind
33124	6	9325	6	NULL	NULL	0	NULL	p53	NULL		inhibits	NULL		carboxy-terminal region		statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_6_9_1057_s_42	8805363	A carboxy-terminal region of p53 binds to XPB and XPD and this region of p53 inhibits their DNA helicase activities    [7,8,10]  .	bind
40201	1	9326	5	13	NULL	NULL	NULL	NusA	GP	 truncated	bind		specifically	carboxy-terminal		RNA	NucleicAcid		nut -site		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_20_2664_s_161	11040219	A carboxy-terminally truncated NusA also binds specifically to nut -site RNA	bind
33125	1	9326	6	10	NULL	0	NULL	NusA	NULL	truncated	bind	NULL	specifically	carboxy terminal		 RNA	NULL		nut -site		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_20_2664_s_161	11040219	A carboxy-terminally truncated NusA also binds specifically to nut -site RNA	bind
40215	1	9327	5	13	NULL	NULL	NULL	lipoprotein lipase	GP		bind			carboxyl-terminal fragment		low density lipoprotein receptor-related protein	GP				NULL	cells	NULL	NULL	NULL	NULL	gw60_jlipidres_39_3_633_s_552	9548595	A carboxyl-terminal fragment of lipoprotein lipase binds to the low density lipoprotein receptor-related protein and inhibits lipase-mediated uptake of lipoprotein in cells.	bind
40216	2	9327	5	13	NULL	NULL	NULL	lipase	GP		mediate					lipoprotein	GP	uptake of			NULL	cells	NULL	NULL	NULL	NULL	gw60_jlipidres_39_3_633_s_552	9548595	A carboxyl-terminal fragment of lipoprotein lipase binds to the low density lipoprotein receptor-related protein and inhibits lipase-mediated uptake of lipoprotein in cells.	bind
40217	3	9327	5	13	NULL	NULL	NULL	statement 1	Process		inhibit					statement 2	Process				NULL	cells	NULL	NULL	NULL	NULL	gw60_jlipidres_39_3_633_s_552	9548595	A carboxyl-terminal fragment of lipoprotein lipase binds to the low density lipoprotein receptor-related protein and inhibits lipase-mediated uptake of lipoprotein in cells.	bind
33127	1	9327	6	10	NULL	0	NULL	lipoprotein lipase			bind			carboxy terminal fragment		low density lipoprotein receptor-related protein					NULL	cells	NULL	NULL	NULL	NULL	gw60_jlipidres_39_3_633_s_552	9548595	A carboxyl-terminal fragment of lipoprotein lipase binds to the low density lipoprotein receptor-related protein and inhibits lipase-mediated uptake of lipoprotein in cells.	bind
33128	2	9327	6	NULL	NULL	0	NULL	lipase	NULL		mediates	NULL				lipoprotein	NULL	uptake of			NULL	cells	0	NULL	NULL	NULL	gw60_jlipidres_39_3_633_s_552	9548595	A carboxyl-terminal fragment of lipoprotein lipase binds to the low density lipoprotein receptor-related protein and inhibits lipase-mediated uptake of lipoprotein in cells.	bind
33131	3	9327	6	10	NULL	0	NULL	statement 1			inhibits					statement 2					NULL	cells	NULL	NULL	NULL	NULL	gw60_jlipidres_39_3_633_s_552	9548595	A carboxyl-terminal fragment of lipoprotein lipase binds to the low density lipoprotein receptor-related protein and inhibits lipase-mediated uptake of lipoprotein in cells.	bind
40219	1	9329	5	13	NULL	NULL	NULL	IKKgamma	GP	 truncated	bind			carboxyl-terminal		IKKalpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29779_s_38	10893415	A carboxyl-terminal truncated IKKgamma, which still binds to IKKalpha and -beta, acts as an inhibitor of cytokine-induced, but not of basal IKK kinase activity, when overexpressed ( 27).	bind
40220	2	9329	5	13	NULL	NULL	NULL	IKKgamma	GP	 truncated	bind			carboxyl-terminal		IKKbeta	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29779_s_38	10893415	A carboxyl-terminal truncated IKKgamma, which still binds to IKKalpha and -beta, acts as an inhibitor of cytokine-induced, but not of basal IKK kinase activity, when overexpressed ( 27).	bind
40222	3	9329	5	13	NULL	NULL	NULL	cytokine	GP		induce					IKK kinase	GP	 activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29779_s_38	10893415	A carboxyl-terminal truncated IKKgamma, which still binds to IKKalpha and -beta, acts as an inhibitor of cytokine-induced, but not of basal IKK kinase activity, when overexpressed ( 27).	bind
40224	4	9329	5	13	NULL	NULL	NULL	IKKgamma	GP	 truncated;;overexpressed	inhibit			carboxyl-terminal		statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29779_s_38	10893415	A carboxyl-terminal truncated IKKgamma, which still binds to IKKalpha and -beta, acts as an inhibitor of cytokine-induced, but not of basal IKK kinase activity, when overexpressed ( 27).	bind
40225	5	9329	5	13	NULL	NULL	NULL	IKKgamma	GP	truncated;;overexpressed	does not inhibit			carboxyl-terminal 		IKK kinase	GP	basal activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29779_s_38	10893415	A carboxyl-terminal truncated IKKgamma, which still binds to IKKalpha and -beta, acts as an inhibitor of cytokine-induced, but not of basal IKK kinase activity, when overexpressed ( 27).	bind
33171	1	9329	6	NULL	NULL	0	NULL	IKKgamma	NULL	truncated	bind	NULL		carboxy terminal		IKKalpha	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29779_s_38	10893415	A carboxyl-terminal truncated IKKgamma, which still binds to IKKalpha and -beta, acts as an inhibitor of cytokine-induced, but not of basal IKK kinase activity, when overexpressed ( 27).	bind
33173	2	9329	6	NULL	NULL	0	NULL	IKKgamma	NULL	truncated	bind	NULL		carboxy terminal		IKKbeta	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29779_s_38	10893415	A carboxyl-terminal truncated IKKgamma, which still binds to IKKalpha and -beta, acts as an inhibitor of cytokine-induced, but not of basal IKK kinase activity, when overexpressed ( 27).	bind
33889	3	9329	6	NULL	NULL	0	NULL	cytokine	NULL		induces	NULL				IKK kinase	NULL	activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29779_s_38	10893415	A carboxyl-terminal truncated IKKgamma, which still binds to IKKalpha and -beta, acts as an inhibitor of cytokine-induced, but not of basal IKK kinase activity, when overexpressed ( 27).	bind
33890	4	9329	6	NULL	NULL	0	NULL	IKKgamma	NULL	truncated	inhibits	NULL		carboxyl-terminal		statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29779_s_38	10893415	A carboxyl-terminal truncated IKKgamma, which still binds to IKKalpha and -beta, acts as an inhibitor of cytokine-induced, but not of basal IKK kinase activity, when overexpressed ( 27).	bind
33891	5	9329	6	10	NULL	0	NULL	IKKgamma	NULL	truncated	does not inhibit	NULL		carboxyl-terminal		IKK kinase	NULL	basal activity of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29779_s_38	10893415	A carboxyl-terminal truncated IKKgamma, which still binds to IKKalpha and -beta, acts as an inhibitor of cytokine-induced, but not of basal IKK kinase activity, when overexpressed ( 27).	bind
40227	1	9330	5	13	NULL	NULL	NULL	CD40	GP	truncation mutant	lacks			carboxyl					last 32 amino acids		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_32_22414_s_7	10428814	A carboxyl-truncation mutant of CD40 lacking the last 32 amino acids required for TRAF2 and TRAF3 binding, CD40(delta32), mediated NF-kappaB induction through a mechanism that was suppressible by co-expression of TRAF6(deltaN), a dominant-negative version of TRAF6, but not by TRAF2(deltaN), implying that while TRAF6 does not directly bind CD40, it can participate in CD40 signaling.	bind
40524	3	9330	5	13	NULL	NULL	NULL	statement 1	GP		is required for					TRAF2	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_32_22414_s_7	10428814	A carboxyl-truncation mutant of CD40 lacking the last 32 amino acids required for TRAF2 and TRAF3 binding, CD40(delta32), mediated NF-kappaB induction through a mechanism that was suppressible by co-expression of TRAF6(deltaN), a dominant-negative version of TRAF6, but not by TRAF2(deltaN), implying that while TRAF6 does not directly bind CD40, it can participate in CD40 signaling.	bind
40525	4	9330	5	13	NULL	NULL	NULL	statement 1	GP		is required for					TRAF3	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_32_22414_s_7	10428814	A carboxyl-truncation mutant of CD40 lacking the last 32 amino acids required for TRAF2 and TRAF3 binding, CD40(delta32), mediated NF-kappaB induction through a mechanism that was suppressible by co-expression of TRAF6(deltaN), a dominant-negative version of TRAF6, but not by TRAF2(deltaN), implying that while TRAF6 does not directly bind CD40, it can participate in CD40 signaling.	bind
40535	2	9330	5	13	NULL	NULL	NULL	CD40(delta32)	GP		is					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_32_22414_s_7	10428814	A carboxyl-truncation mutant of CD40 lacking the last 32 amino acids required for TRAF2 and TRAF3 binding, CD40(delta32), mediated NF-kappaB induction through a mechanism that was suppressible by co-expression of TRAF6(deltaN), a dominant-negative version of TRAF6, but not by TRAF2(deltaN), implying that while TRAF6 does not directly bind CD40, it can participate in CD40 signaling.	bind
40536	5	9330	5	13	NULL	NULL	NULL	CD40(delta32)	GP		mediate					NF-kappaB	GP	induction of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_32_22414_s_7	10428814	A carboxyl-truncation mutant of CD40 lacking the last 32 amino acids required for TRAF2 and TRAF3 binding, CD40(delta32), mediated NF-kappaB induction through a mechanism that was suppressible by co-expression of TRAF6(deltaN), a dominant-negative version of TRAF6, but not by TRAF2(deltaN), implying that while TRAF6 does not directly bind CD40, it can participate in CD40 signaling.	bind
40538	6	9330	5	13	NULL	NULL	NULL	TRAF6(deltaN)	GP		is					dominant-negative version of TRAF6	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_32_22414_s_7	10428814	A carboxyl-truncation mutant of CD40 lacking the last 32 amino acids required for TRAF2 and TRAF3 binding, CD40(delta32), mediated NF-kappaB induction through a mechanism that was suppressible by co-expression of TRAF6(deltaN), a dominant-negative version of TRAF6, but not by TRAF2(deltaN), implying that while TRAF6 does not directly bind CD40, it can participate in CD40 signaling.	bind
40540	7	9330	5	13	NULL	NULL	NULL	TRAF6	GP		does not bind		directly			CD40	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_32_22414_s_7	10428814	A carboxyl-truncation mutant of CD40 lacking the last 32 amino acids required for TRAF2 and TRAF3 binding, CD40(delta32), mediated NF-kappaB induction through a mechanism that was suppressible by co-expression of TRAF6(deltaN), a dominant-negative version of TRAF6, but not by TRAF2(deltaN), implying that while TRAF6 does not directly bind CD40, it can participate in CD40 signaling.	bind
40541	8	9330	5	13	NULL	NULL	NULL	TRAF6	GP		participate in					CD40	GP	signaling of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_32_22414_s_7	10428814	A carboxyl-truncation mutant of CD40 lacking the last 32 amino acids required for TRAF2 and TRAF3 binding, CD40(delta32), mediated NF-kappaB induction through a mechanism that was suppressible by co-expression of TRAF6(deltaN), a dominant-negative version of TRAF6, but not by TRAF2(deltaN), implying that while TRAF6 does not directly bind CD40, it can participate in CD40 signaling.	bind
33892	1	9330	6	NULL	NULL	0	NULL	TRAF6	NULL		does not bind	NULL	directly			CD40	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_32_22414_s_7	10428814	A carboxyl-truncation mutant of CD40 lacking the last 32 amino acids required for TRAF2 and TRAF3 binding, CD40(delta32), mediated NF-kappaB induction through a mechanism that was suppressible by co-expression of TRAF6(deltaN), a dominant-negative version of TRAF6, but not by TRAF2(deltaN), implying that while TRAF6 does not directly bind CD40, it can participate in CD40 signaling.	bind
33893	2	9330	6	NULL	NULL	0	NULL	TRAF6	NULL		can participate	NULL				CD40	NULL	signaling of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_32_22414_s_7	10428814	A carboxyl-truncation mutant of CD40 lacking the last 32 amino acids required for TRAF2 and TRAF3 binding, CD40(delta32), mediated NF-kappaB induction through a mechanism that was suppressible by co-expression of TRAF6(deltaN), a dominant-negative version of TRAF6, but not by TRAF2(deltaN), implying that while TRAF6 does not directly bind CD40, it can participate in CD40 signaling.	bind
33894	3	9330	6	10	NULL	0	NULL	CD40(delta32)			is required for					TRAF2		binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_32_22414_s_7	10428814	A carboxyl-truncation mutant of CD40 lacking the last 32 amino acids required for TRAF2 and TRAF3 binding, CD40(delta32), mediated NF-kappaB induction through a mechanism that was suppressible by co-expression of TRAF6(deltaN), a dominant-negative version of TRAF6, but not by TRAF2(deltaN), implying that while TRAF6 does not directly bind CD40, it can participate in CD40 signaling.	bind
33895	4	9330	6	10	NULL	0	NULL	CD40(delta32)			is required for					TRAF3		binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_32_22414_s_7	10428814	A carboxyl-truncation mutant of CD40 lacking the last 32 amino acids required for TRAF2 and TRAF3 binding, CD40(delta32), mediated NF-kappaB induction through a mechanism that was suppressible by co-expression of TRAF6(deltaN), a dominant-negative version of TRAF6, but not by TRAF2(deltaN), implying that while TRAF6 does not directly bind CD40, it can participate in CD40 signaling.	bind
33896	5	9330	6	10	NULL	0	NULL	CD40(delta32)			mediates					NF-kappaB		induction of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_32_22414_s_7	10428814	A carboxyl-truncation mutant of CD40 lacking the last 32 amino acids required for TRAF2 and TRAF3 binding, CD40(delta32), mediated NF-kappaB induction through a mechanism that was suppressible by co-expression of TRAF6(deltaN), a dominant-negative version of TRAF6, but not by TRAF2(deltaN), implying that while TRAF6 does not directly bind CD40, it can participate in CD40 signaling.	bind
40526	6	9330	6	NULL	NULL	0	NULL	TRAF6(deltaN)	NULL		is	NULL				dominant-negative version of TRAF6	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_32_22414_s_7	10428814	A carboxyl-truncation mutant of CD40 lacking the last 32 amino acids required for TRAF2 and TRAF3 binding, CD40(delta32), mediated NF-kappaB induction through a mechanism that was suppressible by co-expression of TRAF6(deltaN), a dominant-negative version of TRAF6, but not by TRAF2(deltaN), implying that while TRAF6 does not directly bind CD40, it can participate in CD40 signaling.	bind
40527	7	9330	6	NULL	NULL	0	NULL	CD40(delta32)	NULL		is	NULL				carboxyl-truncation mutant of CD40 lacking the last 32 amino acids	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_32_22414_s_7	10428814	A carboxyl-truncation mutant of CD40 lacking the last 32 amino acids required for TRAF2 and TRAF3 binding, CD40(delta32), mediated NF-kappaB induction through a mechanism that was suppressible by co-expression of TRAF6(deltaN), a dominant-negative version of TRAF6, but not by TRAF2(deltaN), implying that while TRAF6 does not directly bind CD40, it can participate in CD40 signaling.	bind
40229	1	9331	5	13	NULL	NULL	NULL				similar to				CArG sequence	c- fos	GP			SRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_410_s_216	7814403	A CArG Box Is Required for Expression of the SkACT  Promoter, but Not the beta-MHC Promoter The CArG sequence is  similar to the c- fos  serum response element (SRE), and both  bind the SRF ( 46 ,  47 ) .	bind
40230	2	9331	5	13	NULL	NULL	NULL	SRE	GP		is					serum response element	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_410_s_216	7814403	A CArG Box Is Required for Expression of the SkACT  Promoter, but Not the beta-MHC Promoter The CArG sequence is  similar to the c- fos  serum response element (SRE), and both  bind the SRF ( 46 ,  47 ) .	bind
40232	3	9331	5	13	NULL	NULL	NULL				bind				CArG sequence	SRF	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_410_s_216	7814403	A CArG Box Is Required for Expression of the SkACT  Promoter, but Not the beta-MHC Promoter The CArG sequence is  similar to the c- fos  serum response element (SRE), and both  bind the SRF ( 46 ,  47 ) .	bind
40233	4	9331	5	13	NULL	NULL	NULL	c- fos	GP		bind				SRE	SRF	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_410_s_216	7814403	A CArG Box Is Required for Expression of the SkACT  Promoter, but Not the beta-MHC Promoter The CArG sequence is  similar to the c- fos  serum response element (SRE), and both  bind the SRF ( 46 ,  47 ) .	bind
40234	5	9331	5	13	NULL	NULL	NULL				is required for				CArG Box	SkACT	NucleicAcid	expression of		promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_410_s_216	7814403	A CArG Box Is Required for Expression of the SkACT  Promoter, but Not the beta-MHC Promoter The CArG sequence is  similar to the c- fos  serum response element (SRE), and both  bind the SRF ( 46 ,  47 ) .	bind
40235	6	9331	5	13	NULL	NULL	NULL				is not required for				CArG Box	beta-MHC	NucleicAcid	expression of		promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_410_s_216	7814403	A CArG Box Is Required for Expression of the SkACT  Promoter, but Not the beta-MHC Promoter The CArG sequence is  similar to the c- fos  serum response element (SRE), and both  bind the SRF ( 46 ,  47 ) .	bind
33184	1	9331	6	NULL	NULL	0	NULL		NULL		is required for	NULL			CArG Box	SkACT	NULL	expression of		promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_410_s_216	7814403	A CArG Box Is Required for Expression of the SkACT  Promoter, but Not the beta-MHC Promoter The CArG sequence is  similar to the c- fos  serum response element (SRE), and both  bind the SRF ( 46 ,  47 ) .	bind
33189	2	9331	6	NULL	NULL	0	NULL	CArG sequence	NULL		is similar to	NULL				c-fos	NULL			SRE	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_410_s_216	7814403	A CArG Box Is Required for Expression of the SkACT  Promoter, but Not the beta-MHC Promoter The CArG sequence is  similar to the c- fos  serum response element (SRE), and both  bind the SRF ( 46 ,  47 ) .	bind
33258	3	9331	6	NULL	NULL	0	NULL		NULL		is not required for	NULL			CArG box	beta-MHC	NULL	expression of		promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_410_s_216	7814403	A CArG Box Is Required for Expression of the SkACT  Promoter, but Not the beta-MHC Promoter The CArG sequence is  similar to the c- fos  serum response element (SRE), and both  bind the SRF ( 46 ,  47 ) .	bind
33259	4	9331	6	NULL	NULL	0	NULL	SRE	NULL		is	NULL				serum response element	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_410_s_216	7814403	A CArG Box Is Required for Expression of the SkACT  Promoter, but Not the beta-MHC Promoter The CArG sequence is  similar to the c- fos  serum response element (SRE), and both  bind the SRF ( 46 ,  47 ) .	bind
33261	5	9331	6	NULL	NULL	0	NULL	c-fos	NULL		bind	NULL			SRE	SRF	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_410_s_216	7814403	A CArG Box Is Required for Expression of the SkACT  Promoter, but Not the beta-MHC Promoter The CArG sequence is  similar to the c- fos  serum response element (SRE), and both  bind the SRF ( 46 ,  47 ) .	bind
33268	6	9331	6	NULL	NULL	0	NULL		NULL		bind	NULL			CArG box	SRF	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_410_s_216	7814403	A CArG Box Is Required for Expression of the SkACT  Promoter, but Not the beta-MHC Promoter The CArG sequence is  similar to the c- fos  serum response element (SRE), and both  bind the SRF ( 46 ,  47 ) .	bind
40238	1	9332	5	13	NULL	NULL	NULL	NES	GP		is					nuclear export signal	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_15_0_291_s_42	10611964	A cargo bearing a nuclear  export signal (NES) binds a soluble export receptor, known as exportin, in the nucleus.	bind
40239	2	9332	5	13	NULL	NULL	NULL	cargo	GP		bind			NES		exportin	GP				NULL	nucleus	NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_15_0_291_s_42	10611964	A cargo bearing a nuclear  export signal (NES) binds a soluble export receptor, known as exportin, in the nucleus.	bind
40241	3	9332	5	13	NULL	NULL	NULL	exportin	GP		is a type of					soluble export receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_15_0_291_s_42	10611964	A cargo bearing a nuclear  export signal (NES) binds a soluble export receptor, known as exportin, in the nucleus.	bind
33271	1	9332	6	NULL	NULL	0	NULL	NES	NULL		is	NULL				nuclear export signal	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevcelldevbiol_15_0_291_s_42	10611964	A cargo bearing a nuclear  export signal (NES) binds a soluble export receptor, known as exportin, in the nucleus.	bind
33272	2	9332	6	10	NULL	0	NULL	exportin	NULL		is a type of	NULL				soluble export receptor	NULL				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_15_0_291_s_42	10611964	A cargo bearing a nuclear  export signal (NES) binds a soluble export receptor, known as exportin, in the nucleus.	bind
33274	3	9332	6	10	NULL	0	NULL	NES cargo			bind					exportin					NULL	nucleus	NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_15_0_291_s_42	10611964	A cargo bearing a nuclear  export signal (NES) binds a soluble export receptor, known as exportin, in the nucleus.	bind
40242	1	9334	5	13	NULL	NULL	NULL	carrier precursor	GP		exits					TOM channel	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_279_5349_369_s_130	9430585	A carrier precursor exiting the TOM channel is captured by Tim10p in the intermembrane space and delivered to Tim12p, which is bound to Tim22p at the outer face of the inner membrane.	bind
40243	2	9334	5	13	NULL	NULL	NULL	statement 1	GP		is captured by					Tim10p	GP				NULL	intermembrane space	NULL	NULL	NULL	NULL	gw60_science_279_5349_369_s_130	9430585	A carrier precursor exiting the TOM channel is captured by Tim10p in the intermembrane space and delivered to Tim12p, which is bound to Tim22p at the outer face of the inner membrane.	bind
40244	4	9334	5	13	NULL	NULL	NULL	statement 2	GP		is delivered to					statement 3	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_279_5349_369_s_130	9430585	A carrier precursor exiting the TOM channel is captured by Tim10p in the intermembrane space and delivered to Tim12p, which is bound to Tim22p at the outer face of the inner membrane.	bind
40245	3	9334	5	13	NULL	NULL	NULL	Tim12p	GP		bind					Tim22p	GP				NULL	outer face of the inner membrane	NULL	NULL	NULL	NULL	gw60_science_279_5349_369_s_130	9430585	A carrier precursor exiting the TOM channel is captured by Tim10p in the intermembrane space and delivered to Tim12p, which is bound to Tim22p at the outer face of the inner membrane.	bind
33277	1	9334	6	NULL	NULL	0	NULL	carrier precursor	NULL		exit 	NULL				TOM channel	NULL				NULL	intermembrane space	NULL	NULL	NULL	NULL	gw60_science_279_5349_369_s_130	9430585	A carrier precursor exiting the TOM channel is captured by Tim10p in the intermembrane space and delivered to Tim12p, which is bound to Tim22p at the outer face of the inner membrane.	bind
33278	2	9334	6	10	NULL	0	NULL	statement 1			is captured by					Tim10p					NULL	intermembrane space	NULL	NULL	NULL	NULL	gw60_science_279_5349_369_s_130	9430585	A carrier precursor exiting the TOM channel is captured by Tim10p in the intermembrane space and delivered to Tim12p, which is bound to Tim22p at the outer face of the inner membrane.	bind
33280	3	9334	6	10	NULL	0	NULL	Tim12p			bind					Tim22p					NULL	outer face of the inner membrane	NULL	NULL	NULL	NULL	gw60_science_279_5349_369_s_130	9430585	A carrier precursor exiting the TOM channel is captured by Tim10p in the intermembrane space and delivered to Tim12p, which is bound to Tim22p at the outer face of the inner membrane.	bind
33281	4	9334	6	10	NULL	0	NULL	statement 2			is delivered to					statement 3					NULL		NULL	NULL	NULL	NULL	gw60_science_279_5349_369_s_130	9430585	A carrier precursor exiting the TOM channel is captured by Tim10p in the intermembrane space and delivered to Tim12p, which is bound to Tim22p at the outer face of the inner membrane.	bind
40246	1	9335	5	13	NULL	NULL	NULL	NGF	GP		bind					TrkA receptors	GP				NULL	medulloblastoma tumor cells	NULL	NULL	NULL	NULL	gw60_jneurosci_18_9_3273_s_296	9547236	A case in point is the demonstration of apoptosis in medulloblastoma tumor cells by NGF binding to TrkA receptors (Muragaki et al., 1997  ).	bind
40247	2	9335	5	13	NULL	NULL	NULL	statement 1	Process		leads to					apoptosis	Process				NULL	medulloblastoma tumor cells	NULL	NULL	NULL	NULL	gw60_jneurosci_18_9_3273_s_296	9547236	A case in point is the demonstration of apoptosis in medulloblastoma tumor cells by NGF binding to TrkA receptors (Muragaki et al., 1997  ).	bind
33282	1	9335	6	10	NULL	0	NULL	NGF	NULL		bind	NULL				TrkA receptors	NULL				NULL	medulloblastoma tumor cells	NULL	NULL	NULL	NULL	gw60_jneurosci_18_9_3273_s_296	9547236	A case in point is the demonstration of apoptosis in medulloblastoma tumor cells by NGF binding to TrkA receptors (Muragaki et al., 1997  ).	bind
33283	2	9335	6	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				apoptosis	NULL				NULL	medulloblastoma tumor cells	0	NULL	NULL	NULL	gw60_jneurosci_18_9_3273_s_296	9547236	A case in point is the demonstration of apoptosis in medulloblastoma tumor cells by NGF binding to TrkA receptors (Muragaki et al., 1997  ).	bind
40248	1	9336	5	13	NULL	NULL	NULL	CARD	GP		is					caspase activation and recruitment domain	GP				NULL		NULL	NULL	NULL	NULL	gw70_nature_430_6996_213_s_32	15190255	A caspase activation and recruitment  domain (CARD) within ASC binds to the caspase-1 prodomain, and overexpression studies  have reported that ASC both promotes and inhibits activation of caspase-1 (refs  4,  7 9).	bind
40249	2	9336	5	13	NULL	NULL	NULL	ASC	GP		bind			CARD		caspase-1	GP		prodomain		NULL		NULL	NULL	NULL	NULL	gw70_nature_430_6996_213_s_32	15190255	A caspase activation and recruitment  domain (CARD) within ASC binds to the caspase-1 prodomain, and overexpression studies  have reported that ASC both promotes and inhibits activation of caspase-1 (refs  4,  7 9).	bind
40250	3	9336	5	13	NULL	NULL	NULL	ASC	GP		promotes					caspase-1	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_nature_430_6996_213_s_32	15190255	A caspase activation and recruitment  domain (CARD) within ASC binds to the caspase-1 prodomain, and overexpression studies  have reported that ASC both promotes and inhibits activation of caspase-1 (refs  4,  7 9).	bind
40251	4	9336	5	13	NULL	NULL	NULL	ASC	GP		inhibit					caspase-1	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_nature_430_6996_213_s_32	15190255	A caspase activation and recruitment  domain (CARD) within ASC binds to the caspase-1 prodomain, and overexpression studies  have reported that ASC both promotes and inhibits activation of caspase-1 (refs  4,  7 9).	bind
33284	1	9336	6	NULL	NULL	0	NULL	ASC	NULL		bind	NULL		CARD		caspase-1	NULL		prodomain		NULL		0	NULL	NULL	NULL	gw70_nature_430_6996_213_s_32	15190255	A caspase activation and recruitment  domain (CARD) within ASC binds to the caspase-1 prodomain, and overexpression studies  have reported that ASC both promotes and inhibits activation of caspase-1 (refs  4,  7 9).	bind
33285	2	9336	6	NULL	NULL	0	NULL	CARD	NULL		is	NULL				caspase activation and recruitment domain	NULL				NULL		0	NULL	NULL	NULL	gw70_nature_430_6996_213_s_32	15190255	A caspase activation and recruitment  domain (CARD) within ASC binds to the caspase-1 prodomain, and overexpression studies  have reported that ASC both promotes and inhibits activation of caspase-1 (refs  4,  7 9).	bind
33286	3	9336	6	NULL	NULL	0	NULL	ASC	NULL		promotes	NULL				caspase-1	NULL	activation of			NULL		0	NULL	NULL	NULL	gw70_nature_430_6996_213_s_32	15190255	A caspase activation and recruitment  domain (CARD) within ASC binds to the caspase-1 prodomain, and overexpression studies  have reported that ASC both promotes and inhibits activation of caspase-1 (refs  4,  7 9).	bind
33287	4	9336	6	NULL	NULL	0	NULL	ASC	NULL		inhibits	NULL				caspase-1	NULL	activation of			NULL		0	NULL	NULL	NULL	gw70_nature_430_6996_213_s_32	15190255	A caspase activation and recruitment  domain (CARD) within ASC binds to the caspase-1 prodomain, and overexpression studies  have reported that ASC both promotes and inhibits activation of caspase-1 (refs  4,  7 9).	bind
40312	1	9339	5	13	NULL	NULL	NULL	Ubc4	GP		is			C86A		Ubc4	GP	catalytically inactive derivative of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4691_s_213	10848595	A catalytically inactive derivative of Ubc4 (Ubc4C86A) can bind the proteasome.	bind
40313	2	9339	5	13	NULL	NULL	NULL	statement 1	GP		bind					proteasome	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4691_s_213	10848595	A catalytically inactive derivative of Ubc4 (Ubc4C86A) can bind the proteasome.	bind
33288	1	9339	6	NULL	NULL	0	NULL	Ubc4	NULL		bind	NULL		C86A		proteasome	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_13_4691_s_213	10848595	A catalytically inactive derivative of Ubc4 (Ubc4C86A) can bind the proteasome.	bind
33289	2	9339	6	NULL	NULL	0	NULL	Ubc4C86A	NULL		is	NULL				catalytically inactive derivative of Ubc4	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_13_4691_s_213	10848595	A catalytically inactive derivative of Ubc4 (Ubc4C86A) can bind the proteasome.	bind
40314	1	9340	5	13	NULL	NULL	NULL	MKP7 C/S	GP		is					catalytically inactive mutant of MKP7	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_12_10731_s_173	12524447	A catalytically inactive mutant of MKP7 (MKP7 C/S) that still binds JIP-1 did not block the JIP-1-mediated enhancement of JNK activation (Fig.  4 A,  lane 10).	bind
40315	2	9340	5	13	NULL	NULL	NULL	MKP7 C/S	GP		bind					JIP-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_12_10731_s_173	12524447	A catalytically inactive mutant of MKP7 (MKP7 C/S) that still binds JIP-1 did not block the JIP-1-mediated enhancement of JNK activation (Fig.  4 A,  lane 10).	bind
40316	3	9340	5	13	NULL	NULL	NULL	JIP-1	GP		mediate					JNK	GP	enhancement of;;activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_12_10731_s_173	12524447	A catalytically inactive mutant of MKP7 (MKP7 C/S) that still binds JIP-1 did not block the JIP-1-mediated enhancement of JNK activation (Fig.  4 A,  lane 10).	bind
40317	4	9340	5	13	NULL	NULL	NULL	statement 2	Process		does not block					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_12_10731_s_173	12524447	A catalytically inactive mutant of MKP7 (MKP7 C/S) that still binds JIP-1 did not block the JIP-1-mediated enhancement of JNK activation (Fig.  4 A,  lane 10).	bind
33290	1	9340	6	NULL	NULL	0	NULL	MKP7 C/S	NULL		bind	NULL				JIP-1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_12_10731_s_173	12524447	A catalytically inactive mutant of MKP7 (MKP7 C/S) that still binds JIP-1 did not block the JIP-1-mediated enhancement of JNK activation (Fig.  4 A,  lane 10).	bind
33291	2	9340	6	NULL	NULL	0	NULL	MKP7 C/S	NULL		is	NULL				catalytically inactive mutant of MKP7	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_12_10731_s_173	12524447	A catalytically inactive mutant of MKP7 (MKP7 C/S) that still binds JIP-1 did not block the JIP-1-mediated enhancement of JNK activation (Fig.  4 A,  lane 10).	bind
33292	3	9340	6	NULL	NULL	0	NULL	JNK	NULL	activation of	is mediated by	NULL				JIP-1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_12_10731_s_173	12524447	A catalytically inactive mutant of MKP7 (MKP7 C/S) that still binds JIP-1 did not block the JIP-1-mediated enhancement of JNK activation (Fig.  4 A,  lane 10).	bind
33293	4	9340	6	NULL	NULL	0	NULL	MKP7 C/S	NULL		did not block	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_12_10731_s_173	12524447	A catalytically inactive mutant of MKP7 (MKP7 C/S) that still binds JIP-1 did not block the JIP-1-mediated enhancement of JNK activation (Fig.  4 A,  lane 10).	bind
40688	1	9341	5	13	NULL	NULL	NULL	Nedd4 construct	GP	catalytically inactive	does not bind					ER	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_4_1978_s_215	16314411	A catalytically inactive Nedd4 construct also failed to bind ER ( Fig. 5 D).	bind
33294	1	9341	6	NULL	NULL	0	NULL	Nedd4 construct	NULL	catalytically inactive	does not bind	NULL				ER	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_4_1978_s_215	16314411	A catalytically inactive Nedd4 construct also failed to bind ER ( Fig. 5 D).	bind
40689	1	9342	5	13	NULL	NULL	NULL	stathmin derivatives	GP	overexpression of truncated	bind					tubulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_25_22718_s_242	11956188	A catastrophe-promoting activity of stathmin has also been postulated ( 40) to explain that overexpression of truncated stathmin derivatives, which bind tubulin less tightly than wild-type stathmin, still results in microtubule destabilization.	bind
40690	2	9342	5	13	NULL	NULL	NULL	stathmin	GP	wild type	bind					tubulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_25_22718_s_242	11956188	A catastrophe-promoting activity of stathmin has also been postulated ( 40) to explain that overexpression of truncated stathmin derivatives, which bind tubulin less tightly than wild-type stathmin, still results in microtubule destabilization.	bind
40691	3	9342	5	13	NULL	NULL	NULL	statement 1	Process	affinity of	is more than					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_25_22718_s_242	11956188	A catastrophe-promoting activity of stathmin has also been postulated ( 40) to explain that overexpression of truncated stathmin derivatives, which bind tubulin less tightly than wild-type stathmin, still results in microtubule destabilization.	bind
40692	4	9342	5	13	NULL	NULL	NULL	statement 1	Process		results in					microtubule	CellComponent	destabilization of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_25_22718_s_242	11956188	A catastrophe-promoting activity of stathmin has also been postulated ( 40) to explain that overexpression of truncated stathmin derivatives, which bind tubulin less tightly than wild-type stathmin, still results in microtubule destabilization.	bind
40693	5	9342	5	13	NULL	NULL	NULL	stathmin	GP		promote					catastrophe activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_25_22718_s_242	11956188	A catastrophe-promoting activity of stathmin has also been postulated ( 40) to explain that overexpression of truncated stathmin derivatives, which bind tubulin less tightly than wild-type stathmin, still results in microtubule destabilization.	bind
33897	1	9342	6	NULL	NULL	0	NULL	stathmin	NULL	wild type	bind	NULL				tubulin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_25_22718_s_242	11956188	A catastrophe-promoting activity of stathmin has also been postulated ( 40) to explain that overexpression of truncated stathmin derivatives, which bind tubulin less tightly than wild-type stathmin, still results in microtubule destabilization.	bind
33899	2	9342	6	NULL	NULL	0	NULL	stathmin derivatives	NULL	truncated	bind	NULL				tubulin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_25_22718_s_242	11956188	A catastrophe-promoting activity of stathmin has also been postulated ( 40) to explain that overexpression of truncated stathmin derivatives, which bind tubulin less tightly than wild-type stathmin, still results in microtubule destabilization.	bind
33900	3	9342	6	NULL	NULL	0	NULL	statement 1	NULL	affinity of	is more than	NULL				statement 2	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_25_22718_s_242	11956188	A catastrophe-promoting activity of stathmin has also been postulated ( 40) to explain that overexpression of truncated stathmin derivatives, which bind tubulin less tightly than wild-type stathmin, still results in microtubule destabilization.	bind
33901	4	9342	6	10	NULL	0	NULL	stathmin derivatives	NULL	overexpression of;; truncated	results in	NULL				microtubule 	NULL	destabilization of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_25_22718_s_242	11956188	A catastrophe-promoting activity of stathmin has also been postulated ( 40) to explain that overexpression of truncated stathmin derivatives, which bind tubulin less tightly than wild-type stathmin, still results in microtubule destabilization.	bind
58464	5	9342	6	10	NULL	0	NULL	stathmin			promote					catastrophe activity					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_25_22718_s_242	11956188	A catastrophe-promoting activity of stathmin has also been postulated ( 40) to explain that overexpression of truncated stathmin derivatives, which bind tubulin less tightly than wild-type stathmin, still results in microtubule destabilization.	bind
40694	1	9343	5	13	NULL	NULL	NULL	lanthanide complex	Chemical	cationic	bind		selectively			insulin receptor peptide fragment	GP	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_org-biomol-chem_4_16_16886086_s_1	16886086	A cationic lanthanide complex binds selectively to phosphorylated tyrosine sites, aiding NMR analysis of the phosphorylated insulin receptor peptide fragment..	bind
33295	1	9343	6	10	NULL	0	NULL	lanthanide complex	NULL	cationic	bind	NULL	selectively			 insulin receptor peptide fragment	NULL	phosphorylated	tyrosine sites		NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_org-biomol-chem_4_16_16886086_s_1	16886086	A cationic lanthanide complex binds selectively to phosphorylated tyrosine sites, aiding NMR analysis of the phosphorylated insulin receptor peptide fragment..	bind
40695	1	9344	5	13	NULL	NULL	NULL	Ste5	GP	mutant	does not bind					Ste7	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1793_s_295	15713635	A caveat to this interpretation is that it is based upon analysis of a mutant of Ste5 that cannot bind Ste7; perhaps Ste7 binding to Ste5 reduces Ste11 dissociation from Ste5.	bind
40696	2	9344	5	13	NULL	NULL	NULL	Ste7	GP		bind					Ste5	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1793_s_295	15713635	A caveat to this interpretation is that it is based upon analysis of a mutant of Ste5 that cannot bind Ste7; perhaps Ste7 binding to Ste5 reduces Ste11 dissociation from Ste5.	bind
40697	3	9344	5	13	NULL	NULL	NULL	Ste11	GP		dissociates from					Ste5	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1793_s_295	15713635	A caveat to this interpretation is that it is based upon analysis of a mutant of Ste5 that cannot bind Ste7; perhaps Ste7 binding to Ste5 reduces Ste11 dissociation from Ste5.	bind
40698	4	9344	5	13	NULL	NULL	NULL	statement 2	Process		reduces					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_1793_s_295	15713635	A caveat to this interpretation is that it is based upon analysis of a mutant of Ste5 that cannot bind Ste7; perhaps Ste7 binding to Ste5 reduces Ste11 dissociation from Ste5.	bind
33296	1	9344	6	NULL	NULL	0	NULL	Ste5	NULL	mutant	does not bind	NULL				Ste7	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_5_1793_s_295	15713635	A caveat to this interpretation is that it is based upon analysis of a mutant of Ste5 that cannot bind Ste7; perhaps Ste7 binding to Ste5 reduces Ste11 dissociation from Ste5.	bind
33297	2	9344	6	NULL	NULL	0	NULL	Ste7	NULL		bind	NULL				Ste5	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_5_1793_s_295	15713635	A caveat to this interpretation is that it is based upon analysis of a mutant of Ste5 that cannot bind Ste7; perhaps Ste7 binding to Ste5 reduces Ste11 dissociation from Ste5.	bind
33298	3	9344	6	NULL	NULL	0	NULL	ste11	NULL		dissociates from	NULL				Ste5	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_5_1793_s_295	15713635	A caveat to this interpretation is that it is based upon analysis of a mutant of Ste5 that cannot bind Ste7; perhaps Ste7 binding to Ste5 reduces Ste11 dissociation from Ste5.	bind
33299	4	9344	6	NULL	NULL	0	NULL	statement 2	NULL		reduces	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_5_1793_s_295	15713635	A caveat to this interpretation is that it is based upon analysis of a mutant of Ste5 that cannot bind Ste7; perhaps Ste7 binding to Ste5 reduces Ste11 dissociation from Ste5.	bind
40699	1	9345	5	13	NULL	NULL	NULL	Galphaq/11	GP	activated	bind					caveolin-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_30211_s_290	10862762	A caveolin-binding Galphaq/11 fragment that selectively blocked the binding of activated Galphaq/11 to caveolin-3 elicited by ACh prevented desensitization of responses mediated by other Gq/11-coupled receptors but not by Gi3-coupled receptors.	bind
40700	2	9345	5	13	NULL	NULL	NULL	Galphaq/11	GP		block		selectively	caveolin-binding fragment		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_30211_s_290	10862762	A caveolin-binding Galphaq/11 fragment that selectively blocked the binding of activated Galphaq/11 to caveolin-3 elicited by ACh prevented desensitization of responses mediated by other Gq/11-coupled receptors but not by Gi3-coupled receptors.	bind
40701	3	9345	5	13	NULL	NULL	NULL	ACh	Chemical		elicits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_30211_s_290	10862762	A caveolin-binding Galphaq/11 fragment that selectively blocked the binding of activated Galphaq/11 to caveolin-3 elicited by ACh prevented desensitization of responses mediated by other Gq/11-coupled receptors but not by Gi3-coupled receptors.	bind
40702	4	9345	5	13	NULL	NULL	NULL	Gq/11-coupled receptors	GP		mediate					responses	Process	desensitization of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_30211_s_290	10862762	A caveolin-binding Galphaq/11 fragment that selectively blocked the binding of activated Galphaq/11 to caveolin-3 elicited by ACh prevented desensitization of responses mediated by other Gq/11-coupled receptors but not by Gi3-coupled receptors.	bind
40703	5	9345	5	13	NULL	NULL	NULL	Gi3-coupled receptors	GP		mediate					responses	Process	desensitization of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_30211_s_290	10862762	A caveolin-binding Galphaq/11 fragment that selectively blocked the binding of activated Galphaq/11 to caveolin-3 elicited by ACh prevented desensitization of responses mediated by other Gq/11-coupled receptors but not by Gi3-coupled receptors.	bind
40704	6	9345	5	13	NULL	NULL	NULL	statement 2	Process		prevents					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_30211_s_290	10862762	A caveolin-binding Galphaq/11 fragment that selectively blocked the binding of activated Galphaq/11 to caveolin-3 elicited by ACh prevented desensitization of responses mediated by other Gq/11-coupled receptors but not by Gi3-coupled receptors.	bind
40705	7	9345	5	13	NULL	NULL	NULL	statement 2	Process		does not prevent					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_30211_s_290	10862762	A caveolin-binding Galphaq/11 fragment that selectively blocked the binding of activated Galphaq/11 to caveolin-3 elicited by ACh prevented desensitization of responses mediated by other Gq/11-coupled receptors but not by Gi3-coupled receptors.	bind
33903	1	9345	6	NULL	NULL	0	NULL	Galphaq/11	NULL	activated	bind	NULL				caveolin-3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_39_30211_s_290	10862762	A caveolin-binding Galphaq/11 fragment that selectively blocked the binding of activated Galphaq/11 to caveolin-3 elicited by ACh prevented desensitization of responses mediated by other Gq/11-coupled receptors but not by Gi3-coupled receptors.	bind
33905	2	9345	6	NULL	NULL	0	NULL	Galphaq/11 fragment	NULL		bind	NULL				caveolin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_39_30211_s_290	10862762	A caveolin-binding Galphaq/11 fragment that selectively blocked the binding of activated Galphaq/11 to caveolin-3 elicited by ACh prevented desensitization of responses mediated by other Gq/11-coupled receptors but not by Gi3-coupled receptors.	bind
33906	3	9345	6	NULL	NULL	0	NULL	ACh	NULL		elicits	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_30211_s_290	10862762	A caveolin-binding Galphaq/11 fragment that selectively blocked the binding of activated Galphaq/11 to caveolin-3 elicited by ACh prevented desensitization of responses mediated by other Gq/11-coupled receptors but not by Gi3-coupled receptors.	bind
33907	4	9345	6	NULL	NULL	0	NULL	statement 2	NULL		blocks	NULL	selectively			statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_39_30211_s_290	10862762	A caveolin-binding Galphaq/11 fragment that selectively blocked the binding of activated Galphaq/11 to caveolin-3 elicited by ACh prevented desensitization of responses mediated by other Gq/11-coupled receptors but not by Gi3-coupled receptors.	bind
58465	5	9345	6	10	NULL	0	NULL	Gq/11-coupled receptors			mediate					responses		desensitization of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_39_30211_s_290	10862762	A caveolin-binding Galphaq/11 fragment that selectively blocked the binding of activated Galphaq/11 to caveolin-3 elicited by ACh prevented desensitization of responses mediated by other Gq/11-coupled receptors but not by Gi3-coupled receptors.	bind
58467	6	9345	6	10	NULL	0	NULL	Gi3-coupled receptors			mediate					responses		desensitization of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_39_30211_s_290	10862762	A caveolin-binding Galphaq/11 fragment that selectively blocked the binding of activated Galphaq/11 to caveolin-3 elicited by ACh prevented desensitization of responses mediated by other Gq/11-coupled receptors but not by Gi3-coupled receptors.	bind
58468	7	9345	6	10	NULL	0	NULL	statement 4			prevents					statement 5					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_39_30211_s_290	10862762	A caveolin-binding Galphaq/11 fragment that selectively blocked the binding of activated Galphaq/11 to caveolin-3 elicited by ACh prevented desensitization of responses mediated by other Gq/11-coupled receptors but not by Gi3-coupled receptors.	bind
58469	8	9345	6	10	NULL	0	NULL	statement 4			does not prevent					statement 6					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_39_30211_s_290	10862762	A caveolin-binding Galphaq/11 fragment that selectively blocked the binding of activated Galphaq/11 to caveolin-3 elicited by ACh prevented desensitization of responses mediated by other Gq/11-coupled receptors but not by Gi3-coupled receptors.	bind
40706	1	9346	5	13	NULL	NULL	NULL	PfEMP1	GP		bind			CD36 binding domain		CD36	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_4_1766_s_205	10677532	A CD36 binding domain has previously been shown to reside in the CIDR domain of PfEMP1 that bind CD36 ( 20,  21).	bind
40707	2	9346	5	13	NULL	NULL	NULL	PfEMP1	GP		reside in			CD36 binding domain		PfEMP1	GP		CIDR domain		NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_4_1766_s_205	10677532	A CD36 binding domain has previously been shown to reside in the CIDR domain of PfEMP1 that bind CD36 ( 20,  21).	bind
33582	1	9346	6	NULL	NULL	0	NULL	PfEMP1	NULL		bind	NULL		CIDR domain		CD36	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_4_1766_s_205	10677532	A CD36 binding domain has previously been shown to reside in the CIDR domain of PfEMP1 that bind CD36 ( 20,  21).	bind
33583	2	9346	6	NULL	NULL	0	NULL	PfEMP1	NULL		contains	NULL		CIDR domain			NULL		CD36 binding domain		NULL		0	NULL	NULL	NULL	gw60_pnas_97_4_1766_s_205	10677532	A CD36 binding domain has previously been shown to reside in the CIDR domain of PfEMP1 that bind CD36 ( 20,  21).	bind
40708	1	9347	5	13	NULL	NULL	NULL	AC-25	Cell		is a type of					CD4+ T cell clone	Cell				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_36_13279_s_63	15331779	A CD4+ T cell clone (AC-25) isolated from an individual acutely infected with HIV-1 recognizes an antigen derived from the HIV Gag (p24) protein bound to the human class II MHC protein HLA-DR1.	bind
40709	2	9347	5	13	NULL	NULL	NULL	AC-25	Cell		isolated from					individual infected with HIV-1	Organism	acutely 			NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_36_13279_s_63	15331779	A CD4+ T cell clone (AC-25) isolated from an individual acutely infected with HIV-1 recognizes an antigen derived from the HIV Gag (p24) protein bound to the human class II MHC protein HLA-DR1.	bind
40710	3	9347	5	13	NULL	NULL	NULL	Gag  protein	GP	HIV	bind					HLA-DR1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_36_13279_s_63	15331779	A CD4+ T cell clone (AC-25) isolated from an individual acutely infected with HIV-1 recognizes an antigen derived from the HIV Gag (p24) protein bound to the human class II MHC protein HLA-DR1.	bind
40711	4	9347	5	13	NULL	NULL	NULL	HLA-DR1	GP		is a type of					human class II MHC protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_36_13279_s_63	15331779	A CD4+ T cell clone (AC-25) isolated from an individual acutely infected with HIV-1 recognizes an antigen derived from the HIV Gag (p24) protein bound to the human class II MHC protein HLA-DR1.	bind
40712	6	9347	5	13	NULL	NULL	NULL	antigen	GP		derived from					HIV Gag protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_36_13279_s_63	15331779	A CD4+ T cell clone (AC-25) isolated from an individual acutely infected with HIV-1 recognizes an antigen derived from the HIV Gag (p24) protein bound to the human class II MHC protein HLA-DR1.	bind
48115	5	9347	5	13	NULL	NULL	NULL	Gag protein	GP		is					p24	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_36_13279_s_63	15331779	A CD4+ T cell clone (AC-25) isolated from an individual acutely infected with HIV-1 recognizes an antigen derived from the HIV Gag (p24) protein bound to the human class II MHC protein HLA-DR1.	bind
48117	7	9347	5	13	NULL	NULL	NULL	statement 2	Cell		recognize					statement 6	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_36_13279_s_63	15331779	A CD4+ T cell clone (AC-25) isolated from an individual acutely infected with HIV-1 recognizes an antigen derived from the HIV Gag (p24) protein bound to the human class II MHC protein HLA-DR1.	bind
33584	1	9347	6	NULL	NULL	0	NULL	Gag	NULL	HIV	bind	NULL				HLA-DR1	NULL	human			NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_36_13279_s_63	15331779	A CD4+ T cell clone (AC-25) isolated from an individual acutely infected with HIV-1 recognizes an antigen derived from the HIV Gag (p24) protein bound to the human class II MHC protein HLA-DR1.	bind
33585	2	9347	6	NULL	NULL	0	NULL	HLA-DR1	NULL	human	is a type of	NULL				class II MHC protein	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_101_36_13279_s_63	15331779	A CD4+ T cell clone (AC-25) isolated from an individual acutely infected with HIV-1 recognizes an antigen derived from the HIV Gag (p24) protein bound to the human class II MHC protein HLA-DR1.	bind
33681	3	9347	6	NULL	NULL	0	NULL	Gag	NULL		is	NULL				p24 	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_101_36_13279_s_63	15331779	A CD4+ T cell clone (AC-25) isolated from an individual acutely infected with HIV-1 recognizes an antigen derived from the HIV Gag (p24) protein bound to the human class II MHC protein HLA-DR1.	bind
48116	4	9347	6	10	NULL	0	NULL	AC-25	NULL		is a type of	NULL				CD4+ T cell clone	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_101_36_13279_s_63	15331779	A CD4+ T cell clone (AC-25) isolated from an individual acutely infected with HIV-1 recognizes an antigen derived from the HIV Gag (p24) protein bound to the human class II MHC protein HLA-DR1.	bind
40713	1	9348	5	13	NULL	NULL	NULL	CD44	GP		interact with		indirect;;may			alpha2beta1integrin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_42_43503_s_312	15292257	A CD44/alpha2beta1 integrin interaction may be indirect, because the CD44 cytoplasmic domain binds to ankyrin, which in turn is linked to actin by fodrin/spectrin ( ,  ).	bind
40714	2	9348	5	13	NULL	NULL	NULL	CD44	GP		bind			cytoplasmic domain		ankyrin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_42_43503_s_312	15292257	A CD44/alpha2beta1 integrin interaction may be indirect, because the CD44 cytoplasmic domain binds to ankyrin, which in turn is linked to actin by fodrin/spectrin ( ,  ).	bind
40715	3	9348	5	13	NULL	NULL	NULL	ankyrin	GP		is linked to			cytoplasmic domain		actin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_42_43503_s_312	15292257	A CD44/alpha2beta1 integrin interaction may be indirect, because the CD44 cytoplasmic domain binds to ankyrin, which in turn is linked to actin by fodrin/spectrin ( ,  ).	bind
40716	4	9348	5	13	NULL	NULL	NULL	statement 3	Process		via					fodrin/spectrin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_42_43503_s_312	15292257	A CD44/alpha2beta1 integrin interaction may be indirect, because the CD44 cytoplasmic domain binds to ankyrin, which in turn is linked to actin by fodrin/spectrin ( ,  ).	bind
48118	5	9348	5	13	NULL	NULL	NULL	statement 1	Process		because of					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_42_43503_s_312	15292257	A CD44/alpha2beta1 integrin interaction may be indirect, because the CD44 cytoplasmic domain binds to ankyrin, which in turn is linked to actin by fodrin/spectrin ( ,  ).	bind
33682	1	9348	6	NULL	NULL	0	NULL	CD44	NULL		bind	NULL		cytoplasmic domain		ankyrin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_42_43503_s_312	15292257	A CD44/alpha2beta1 integrin interaction may be indirect, because the CD44 cytoplasmic domain binds to ankyrin, which in turn is linked to actin by fodrin/spectrin ( ,  ).	bind
33683	2	9348	6	NULL	NULL	0	NULL	CD44	NULL		is linked to	NULL		cytoplasmic domain		actin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_42_43503_s_312	15292257	A CD44/alpha2beta1 integrin interaction may be indirect, because the CD44 cytoplasmic domain binds to ankyrin, which in turn is linked to actin by fodrin/spectrin ( ,  ).	bind
33684	3	9348	6	NULL	NULL	0	NULL	statement 2	NULL		occurs by	NULL				fodrin/spectrin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_42_43503_s_312	15292257	A CD44/alpha2beta1 integrin interaction may be indirect, because the CD44 cytoplasmic domain binds to ankyrin, which in turn is linked to actin by fodrin/spectrin ( ,  ).	bind
33685	4	9348	6	NULL	NULL	0	NULL	CD44	NULL		interacts with	NULL	may;; indirectly			alpha2beta1 integrin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_42_43503_s_312	15292257	A CD44/alpha2beta1 integrin interaction may be indirect, because the CD44 cytoplasmic domain binds to ankyrin, which in turn is linked to actin by fodrin/spectrin ( ,  ).	bind
33686	5	9348	6	NULL	NULL	0	NULL	statement 4	NULL		is because of	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_42_43503_s_312	15292257	A CD44/alpha2beta1 integrin interaction may be indirect, because the CD44 cytoplasmic domain binds to ankyrin, which in turn is linked to actin by fodrin/spectrin ( ,  ).	bind
40717	1	9349	5	13	NULL	NULL	NULL	CD8 variant	GP		contains					CDR-2-like loop	GP	mutations in	Q54E/N55D		NULL		NULL	NULL	NULL	NULL	gw60_immunity_10_2_219_s_18	10072074	A CD8   variant with mutations in the CDR-2-like loop (Q54E/N55D), which contacts the  3 domain of HLA-A2 (  Giblin et al. 1994  ; Gao et al. 1997  ), did not bind HLA-A2 (  Figure 1B), confirming the specificity of this interaction.	bind
40718	2	9349	5	13	NULL	NULL	NULL	statement 1	GP		contacts					HLA-A2	GP		3 domain		NULL		NULL	NULL	NULL	NULL	gw60_immunity_10_2_219_s_18	10072074	A CD8   variant with mutations in the CDR-2-like loop (Q54E/N55D), which contacts the  3 domain of HLA-A2 (  Giblin et al. 1994  ; Gao et al. 1997  ), did not bind HLA-A2 (  Figure 1B), confirming the specificity of this interaction.	bind
40719	3	9349	5	13	NULL	NULL	NULL	statement 1	GP		does not bind					HLA-A2	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_10_2_219_s_18	10072074	A CD8   variant with mutations in the CDR-2-like loop (Q54E/N55D), which contacts the  3 domain of HLA-A2 (  Giblin et al. 1994  ; Gao et al. 1997  ), did not bind HLA-A2 (  Figure 1B), confirming the specificity of this interaction.	bind
33908	1	9349	6	10	NULL	0	NULL	CD8 variant			contains							mutation in	 CDR-2-like loop (Q54E/N55D)		NULL		NULL	NULL	NULL	NULL	gw60_immunity_10_2_219_s_18	10072074	A CD8   variant with mutations in the CDR-2-like loop (Q54E/N55D), which contacts the  3 domain of HLA-A2 (  Giblin et al. 1994  ; Gao et al. 1997  ), did not bind HLA-A2 (  Figure 1B), confirming the specificity of this interaction.	bind
33909	2	9349	6	10	NULL	0	NULL	statement 1			contacts					HLA-A2			3 domain		NULL		NULL	NULL	NULL	NULL	gw60_immunity_10_2_219_s_18	10072074	A CD8   variant with mutations in the CDR-2-like loop (Q54E/N55D), which contacts the  3 domain of HLA-A2 (  Giblin et al. 1994  ; Gao et al. 1997  ), did not bind HLA-A2 (  Figure 1B), confirming the specificity of this interaction.	bind
58470	3	9349	6	10	NULL	0	NULL	statement 1			does not bind					HLA-A2					NULL		0	NULL	NULL	NULL	gw60_immunity_10_2_219_s_18	10072074	A CD8   variant with mutations in the CDR-2-like loop (Q54E/N55D), which contacts the  3 domain of HLA-A2 (  Giblin et al. 1994  ; Gao et al. 1997  ), did not bind HLA-A2 (  Figure 1B), confirming the specificity of this interaction.	bind
40722	1	9350	5	13	NULL	NULL	NULL	CD95-IgG antibody	GP		bind					CD95 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_288_2_613_s_118	9918566	A CD95-IgG antibody, which binds to the CD95 receptor without inducing apoptosis, could not prevent the effect of AKBA when the cells were preincubated with this antibody (data not shown).	bind
40723	2	9350	5	13	NULL	NULL	NULL	statement 1	Process		does not induce					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_288_2_613_s_118	9918566	A CD95-IgG antibody, which binds to the CD95 receptor without inducing apoptosis, could not prevent the effect of AKBA when the cells were preincubated with this antibody (data not shown).	bind
40724	3	9350	5	13	NULL	NULL	NULL	statement 1	Process		does not prevent					AKBA	Chemical	effect of			NULL	cells preincubated with CD95-IgG antibody	NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_288_2_613_s_118	9918566	A CD95-IgG antibody, which binds to the CD95 receptor without inducing apoptosis, could not prevent the effect of AKBA when the cells were preincubated with this antibody (data not shown).	bind
33687	1	9350	6	NULL	NULL	0	NULL	CD95-IgG antibody	NULL		bind	NULL				CD95 receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_288_2_613_s_118	9918566	A CD95-IgG antibody, which binds to the CD95 receptor without inducing apoptosis, could not prevent the effect of AKBA when the cells were preincubated with this antibody (data not shown).	bind
33688	2	9350	6	10	NULL	0	NULL	statement 1	NULL		does not induce	NULL				apoptosis	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_288_2_613_s_118	9918566	A CD95-IgG antibody, which binds to the CD95 receptor without inducing apoptosis, could not prevent the effect of AKBA when the cells were preincubated with this antibody (data not shown).	bind
48119	3	9350	6	10	NULL	0	NULL	statement 1	NULL		does not prevent 	NULL				AKBA	NULL	effect of			NULL	cells preincubated with CD95-IgG antibody	0	NULL	NULL	NULL	gw60_jpharmacolexpther_288_2_613_s_118	9918566	A CD95-IgG antibody, which binds to the CD95 receptor without inducing apoptosis, could not prevent the effect of AKBA when the cells were preincubated with this antibody (data not shown).	bind
40725	1	9351	5	13	NULL	NULL	NULL	Cdc20P1	GP		is					Cdc20 peptide	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_15_3133_s_187	15257285	A Cdc20 peptide (Cdc20P1) containing the Mad2-binding motif of Cdc20 bound to N2-Mad2R133A with a dissociation constant ( Kd) of 0.65 muM ( Figure 6C and D).	bind
40726	2	9351	5	13	NULL	NULL	NULL	Cdc20P1	GP		bind			Mad2-binding motif		N2-Mad2	GP		R133A		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_15_3133_s_187	15257285	A Cdc20 peptide (Cdc20P1) containing the Mad2-binding motif of Cdc20 bound to N2-Mad2R133A with a dissociation constant ( Kd) of 0.65 muM ( Figure 6C and D).	bind
33689	1	9351	6	NULL	NULL	0	NULL	Cdc20P1	NULL		is	NULL				Cdc20 peptide	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_23_15_3133_s_187	15257285	A Cdc20 peptide (Cdc20P1) containing the Mad2-binding motif of Cdc20 bound to N2-Mad2R133A with a dissociation constant ( Kd) of 0.65 muM ( Figure 6C and D).	bind
33690	2	9351	6	10	NULL	0	NULL	Cdc20P1			bind			Mad2-binding motif		N2-Mad2			R133A		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_15_3133_s_187	15257285	A Cdc20 peptide (Cdc20P1) containing the Mad2-binding motif of Cdc20 bound to N2-Mad2R133A with a dissociation constant ( Kd) of 0.65 muM ( Figure 6C and D).	bind
40727	1	9352	5	13	NULL	NULL	NULL	SPF1 cDNA	NucleicAcid	sweet potato petiole	bind									SP8 motif	NULL		NULL	NULL	NULL	NULL	gw70_annurevplantbiol_51_0_49_s_350	null	A cDNA clone encoding a new type of DNA-binding protein, SPF1, that binds the SP8  motif was isolated from a sweet potato petiole cDNA library ( 71).	bind
40728	2	9352	5	13	NULL	NULL	NULL	SPF1	GP		is a type of					DNA-binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevplantbiol_51_0_49_s_350	null	A cDNA clone encoding a new type of DNA-binding protein, SPF1, that binds the SP8  motif was isolated from a sweet potato petiole cDNA library ( 71).	bind
33691	1	9352	6	10	NULL	0	NULL	SPF1		sweet potato petiole	bind									SP8 motif	NULL		NULL	NULL	NULL	NULL	gw70_annurevplantbiol_51_0_49_s_350	null	A cDNA clone encoding a new type of DNA-binding protein, SPF1, that binds the SP8  motif was isolated from a sweet potato petiole cDNA library ( 71).	bind
48120	2	9352	6	10	NULL	0	NULL	SPF1	NULL		is a type of	NULL				DNA-binding protein	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevplantbiol_51_0_49_s_350	null	A cDNA clone encoding a new type of DNA-binding protein, SPF1, that binds the SP8  motif was isolated from a sweet potato petiole cDNA library ( 71).	bind
40729	1	9354	5	13	NULL	NULL	NULL	RA	Chemical		induce					RACK1 gene	GP				NULL	chick wing bud	NULL	NULL	NULL	NULL	gw60_development_128_13_2451_s_4	11493562	A cDNA encoding RACK1, a protein that binds and stabilizes activated protein kinase C (PKC), was isolated in a screen for genes induced by retinoic acid (RA) in the chick wing bud.	bind
40730	2	9354	5	13	NULL	NULL	NULL	RACK1 protein	GP		bind					PKC	GP	activated			NULL		NULL	NULL	NULL	NULL	gw60_development_128_13_2451_s_4	11493562	A cDNA encoding RACK1, a protein that binds and stabilizes activated protein kinase C (PKC), was isolated in a screen for genes induced by retinoic acid (RA) in the chick wing bud.	bind
40731	3	9354	5	13	NULL	NULL	NULL	statement 2	Process		stabilize					PKC	GP	activated			NULL		NULL	NULL	NULL	NULL	gw60_development_128_13_2451_s_4	11493562	A cDNA encoding RACK1, a protein that binds and stabilizes activated protein kinase C (PKC), was isolated in a screen for genes induced by retinoic acid (RA) in the chick wing bud.	bind
40732	4	9354	5	13	NULL	NULL	NULL	PKC	GP		is					protein kinase C	GP				NULL		NULL	NULL	NULL	NULL	gw60_development_128_13_2451_s_4	11493562	A cDNA encoding RACK1, a protein that binds and stabilizes activated protein kinase C (PKC), was isolated in a screen for genes induced by retinoic acid (RA) in the chick wing bud.	bind
40733	5	9354	5	13	NULL	NULL	NULL	RA	Chemical		is					retinoic acid	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_development_128_13_2451_s_4	11493562	A cDNA encoding RACK1, a protein that binds and stabilizes activated protein kinase C (PKC), was isolated in a screen for genes induced by retinoic acid (RA) in the chick wing bud.	bind
33692	1	9354	6	NULL	NULL	0	NULL	RACK1	NULL		bind	NULL				PKC	NULL				NULL		0	NULL	NULL	NULL	gw60_development_128_13_2451_s_4	11493562	A cDNA encoding RACK1, a protein that binds and stabilizes activated protein kinase C (PKC), was isolated in a screen for genes induced by retinoic acid (RA) in the chick wing bud.	bind
33693	2	9354	6	NULL	NULL	0	NULL	RACK1	NULL		stabilizes	NULL				PKC	NULL				NULL		0	NULL	NULL	NULL	gw60_development_128_13_2451_s_4	11493562	A cDNA encoding RACK1, a protein that binds and stabilizes activated protein kinase C (PKC), was isolated in a screen for genes induced by retinoic acid (RA) in the chick wing bud.	bind
33694	3	9354	6	NULL	NULL	0	NULL	PKC	NULL		is	NULL				protein kinase C	NULL				NULL		0	NULL	NULL	NULL	gw60_development_128_13_2451_s_4	11493562	A cDNA encoding RACK1, a protein that binds and stabilizes activated protein kinase C (PKC), was isolated in a screen for genes induced by retinoic acid (RA) in the chick wing bud.	bind
48121	4	9354	6	10	NULL	0	NULL	RA	NULL		is	NULL				retinoic acid	NULL				NULL		0	NULL	NULL	NULL	gw60_development_128_13_2451_s_4	11493562	A cDNA encoding RACK1, a protein that binds and stabilizes activated protein kinase C (PKC), was isolated in a screen for genes induced by retinoic acid (RA) in the chick wing bud.	bind
58471	5	9354	6	10	NULL	0	NULL	RA			induce					RACK1 genes					NULL	chick wing bud	0	NULL	NULL	NULL	gw60_development_128_13_2451_s_4	11493562	A cDNA encoding RACK1, a protein that binds and stabilizes activated protein kinase C (PKC), was isolated in a screen for genes induced by retinoic acid (RA) in the chick wing bud.	bind
41257	1	9358	5	13	NULL	NULL	NULL	PBP10	GP		is a type of					cell permeable peptide	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochem-pharmacol_71_10_16549058_s_9	16549058	A cell permeable peptide (PBP10) corresponding to the phosphatidyl-inositol-bisphosphate  binding region of gelsolin, inhibited the FPRL1-, but not the FPR-induced  cellular response and induced the same type of receptor switch.	bind
41258	2	9358	5	13	NULL	NULL	NULL	PBP10	GP		corresponds to					gelsolin	GP		phosphatidyl-inositol-bisphosphate binding region		NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochem-pharmacol_71_10_16549058_s_9	16549058	A cell permeable peptide (PBP10) corresponding to the phosphatidyl-inositol-bisphosphate  binding region of gelsolin, inhibited the FPRL1-, but not the FPR-induced  cellular response and induced the same type of receptor switch.	bind
41259	3	9358	5	13	NULL	NULL	NULL	FPRL1	GP		induce					cellular response	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochem-pharmacol_71_10_16549058_s_9	16549058	A cell permeable peptide (PBP10) corresponding to the phosphatidyl-inositol-bisphosphate  binding region of gelsolin, inhibited the FPRL1-, but not the FPR-induced  cellular response and induced the same type of receptor switch.	bind
41260	4	9358	5	13	NULL	NULL	NULL	PBP10	GP		inhibit					statement 3	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochem-pharmacol_71_10_16549058_s_9	16549058	A cell permeable peptide (PBP10) corresponding to the phosphatidyl-inositol-bisphosphate  binding region of gelsolin, inhibited the FPRL1-, but not the FPR-induced  cellular response and induced the same type of receptor switch.	bind
41261	5	9358	5	13	NULL	NULL	NULL	FPR	GP		induce					cellular response	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochem-pharmacol_71_10_16549058_s_9	16549058	A cell permeable peptide (PBP10) corresponding to the phosphatidyl-inositol-bisphosphate  binding region of gelsolin, inhibited the FPRL1-, but not the FPR-induced  cellular response and induced the same type of receptor switch.	bind
41262	6	9358	5	13	NULL	NULL	NULL	PBP10	GP		does not inhibit					statement 5	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochem-pharmacol_71_10_16549058_s_9	16549058	A cell permeable peptide (PBP10) corresponding to the phosphatidyl-inositol-bisphosphate  binding region of gelsolin, inhibited the FPRL1-, but not the FPR-induced  cellular response and induced the same type of receptor switch.	bind
41263	7	9358	5	13	NULL	NULL	NULL	PBP10	GP		induce					receptor switch	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochem-pharmacol_71_10_16549058_s_9	16549058	A cell permeable peptide (PBP10) corresponding to the phosphatidyl-inositol-bisphosphate  binding region of gelsolin, inhibited the FPRL1-, but not the FPR-induced  cellular response and induced the same type of receptor switch.	bind
33695	1	9358	6	10	NULL	0	NULL	PBP10	NULL		is a type of	NULL				cell permeable peptide	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochem-pharmacol_71_10_16549058_s_9	16549058	A cell permeable peptide (PBP10) corresponding to the phosphatidyl-inositol-bisphosphate  binding region of gelsolin, inhibited the FPRL1-, but not the FPR-induced  cellular response and induced the same type of receptor switch.	bind
33910	2	9358	6	NULL	NULL	0	NULL	FPRL1	NULL		induces	NULL				cellular response	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_biochem-pharmacol_71_10_16549058_s_9	16549058	A cell permeable peptide (PBP10) corresponding to the phosphatidyl-inositol-bisphosphate  binding region of gelsolin, inhibited the FPRL1-, but not the FPR-induced  cellular response and induced the same type of receptor switch.	bind
33911	3	9358	6	NULL	NULL	0	NULL	FPR	NULL		induces	NULL				cellular response	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_biochem-pharmacol_71_10_16549058_s_9	16549058	A cell permeable peptide (PBP10) corresponding to the phosphatidyl-inositol-bisphosphate  binding region of gelsolin, inhibited the FPRL1-, but not the FPR-induced  cellular response and induced the same type of receptor switch.	bind
33912	4	9358	6	NULL	NULL	0	NULL	PBP10	NULL		corresponds to	NULL				gelsolin	NULL		phosphatidyl-inositol-bisphosphate binding region		NULL		0	NULL	NULL	NULL	abs-batch0650-0679_biochem-pharmacol_71_10_16549058_s_9	16549058	A cell permeable peptide (PBP10) corresponding to the phosphatidyl-inositol-bisphosphate  binding region of gelsolin, inhibited the FPRL1-, but not the FPR-induced  cellular response and induced the same type of receptor switch.	bind
33913	5	9358	6	NULL	NULL	0	NULL	PBP10	NULL		inhibits	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_biochem-pharmacol_71_10_16549058_s_9	16549058	A cell permeable peptide (PBP10) corresponding to the phosphatidyl-inositol-bisphosphate  binding region of gelsolin, inhibited the FPRL1-, but not the FPR-induced  cellular response and induced the same type of receptor switch.	bind
33914	6	9358	6	NULL	NULL	0	NULL	PBP10	NULL		does not inhibit	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_biochem-pharmacol_71_10_16549058_s_9	16549058	A cell permeable peptide (PBP10) corresponding to the phosphatidyl-inositol-bisphosphate  binding region of gelsolin, inhibited the FPRL1-, but not the FPR-induced  cellular response and induced the same type of receptor switch.	bind
48122	7	9358	6	10	NULL	0	NULL	PBP10	NULL		induce	NULL				receptor switch	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_biochem-pharmacol_71_10_16549058_s_9	16549058	A cell permeable peptide (PBP10) corresponding to the phosphatidyl-inositol-bisphosphate  binding region of gelsolin, inhibited the FPRL1-, but not the FPR-induced  cellular response and induced the same type of receptor switch.	bind
41255	1	9360	5	13	NULL	NULL	NULL	hsp70	GP		effect		cell type-specific			growth	Process	inhibition of			NULL	transgenic mice expressing hsp70	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7146_s_485	10982831	A cell type-specific effect of hsp70 on growth inhibition was observed in transgenic mice expressing hsp70 under the control of the mouse H-2K promoter ( 28).	bind
41256	2	9360	5	13	NULL	NULL	NULL	statement 1	Process		occurs under 					H-2K	NucleicAcid	control of;;mouse		promoter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7146_s_485	10982831	A cell type-specific effect of hsp70 on growth inhibition was observed in transgenic mice expressing hsp70 under the control of the mouse H-2K promoter ( 28).	bind
33696	1	9360	6	10	NULL	0	NULL	hsp70			effects		cell type-specific			growth 		inhibition of			NULL	transgenic mice	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7146_s_485	10982831	A cell type-specific effect of hsp70 on growth inhibition was observed in transgenic mice expressing hsp70 under the control of the mouse H-2K promoter ( 28).	bind
48123	2	9360	6	10	NULL	0	NULL	statement 1	NULL		occurs under	NULL				H-2K	NULL	control of;;mouse		promoter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_19_7146_s_485	10982831	A cell type-specific effect of hsp70 on growth inhibition was observed in transgenic mice expressing hsp70 under the control of the mouse H-2K promoter ( 28).	bind
40734	1	9361	5	13	NULL	NULL	NULL	mAb 12G5	GP		bind					CXCR4-expressing cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1723_1_270_s_62	15823507	A cell-based ELISA was used for measuring the inhibitory activity of compounds on  the binding of mAb 12G5 to CXCR4-expressing cells   [26].	bind
33697	1	9361	6	NULL	NULL	0	NULL	mAb 12G5	NULL		bind	NULL				CXCR4-expressing cells	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1723_1_270_s_62	15823507	A cell-based ELISA was used for measuring the inhibitory activity of compounds on  the binding of mAb 12G5 to CXCR4-expressing cells   [26].	bind
40735	1	9362	5	13	NULL	NULL	NULL	AR	GP		bind					E2	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_10_5527_s_94	9576916	A cell-free  in vitro transcription/translation system was used to test whether ARA70 can either bind to E2 or increase the AR binding to E2.	bind
33698	1	9362	6	NULL	NULL	0	NULL	AR	NULL		bind	NULL				E2	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_10_5527_s_94	9576916	A cell-free  in vitro transcription/translation system was used to test whether ARA70 can either bind to E2 or increase the AR binding to E2.	bind
40736	1	9363	5	13	NULL	NULL	NULL	RBP	GP		bind					Notch-1	GP		IC		NULL		NULL	NULL	NULL	NULL	gw60_embo_21_20_5417_s_76	12374742	A cell-free synthesized SHARP fragment lacking the RBP-binding site did not reduce RBP binding to Notch-1-IC (lane 12).	bind
40737	2	9363	5	13	NULL	NULL	NULL	SHARP fragment	GP	cell-free synthesized	lacks								RBP-binding site		NULL		NULL	NULL	NULL	NULL	gw60_embo_21_20_5417_s_76	12374742	A cell-free synthesized SHARP fragment lacking the RBP-binding site did not reduce RBP binding to Notch-1-IC (lane 12).	bind
40738	3	9363	5	13	NULL	NULL	NULL	statement 2	Process		does not reduce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_20_5417_s_76	12374742	A cell-free synthesized SHARP fragment lacking the RBP-binding site did not reduce RBP binding to Notch-1-IC (lane 12).	bind
33699	1	9363	6	10	NULL	0	NULL	RBP	NULL		bind	NULL				Notch-1	NULL		IC		NULL		NULL	NULL	NULL	NULL	gw60_embo_21_20_5417_s_76	12374742	A cell-free synthesized SHARP fragment lacking the RBP-binding site did not reduce RBP binding to Notch-1-IC (lane 12).	bind
33700	2	9363	6	10	NULL	0	NULL	SHARP fragment	cell-free synthesized		lacks 								RBP binding site		NULL		NULL	NULL	NULL	NULL	gw60_embo_21_20_5417_s_76	12374742	A cell-free synthesized SHARP fragment lacking the RBP-binding site did not reduce RBP binding to Notch-1-IC (lane 12).	bind
33701	3	9363	6	NULL	NULL	0	NULL	statement 2	NULL		did not reduce	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_21_20_5417_s_76	12374742	A cell-free synthesized SHARP fragment lacking the RBP-binding site did not reduce RBP binding to Notch-1-IC (lane 12).	bind
40739	1	9364	5	13	NULL	NULL	NULL	cell-permeable peptide	GP		is derived from					epidermal growth factor receptor	GP		Grb2-binding sequence		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_18081_s_207	10364261	A cell-permeable peptide derived from the Grb2-binding sequence of epidermal growth factor receptor was shown to inhibit MAP kinase activation in cells stimulated with epidermal growth factor or with platelet-derived growth factor, but not in cells stimulated with bFGF.	bind
40740	2	9364	5	13	NULL	NULL	NULL	statement 1	GP		inhibit					MAP kinase	GP	activation of			NULL	cells stimulated with epidermal growth factor	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_18081_s_207	10364261	A cell-permeable peptide derived from the Grb2-binding sequence of epidermal growth factor receptor was shown to inhibit MAP kinase activation in cells stimulated with epidermal growth factor or with platelet-derived growth factor, but not in cells stimulated with bFGF.	bind
40741	3	9364	5	13	NULL	NULL	NULL	statement 1	GP		inhibit					MAP kinase	GP	activation of			NULL	cells stimulated with platelet-derived growth factor	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_18081_s_207	10364261	A cell-permeable peptide derived from the Grb2-binding sequence of epidermal growth factor receptor was shown to inhibit MAP kinase activation in cells stimulated with epidermal growth factor or with platelet-derived growth factor, but not in cells stimulated with bFGF.	bind
40742	4	9364	5	13	NULL	NULL	NULL	statement 1	GP		does not inhibit					MAP kinase	GP	activation of			NULL	cells stimulated with bFGF	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_18081_s_207	10364261	A cell-permeable peptide derived from the Grb2-binding sequence of epidermal growth factor receptor was shown to inhibit MAP kinase activation in cells stimulated with epidermal growth factor or with platelet-derived growth factor, but not in cells stimulated with bFGF.	bind
40755	5	9364	5	13	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_18081_s_207	10364261	A cell-permeable peptide derived from the Grb2-binding sequence of epidermal growth factor receptor was shown to inhibit MAP kinase activation in cells stimulated with epidermal growth factor or with platelet-derived growth factor, but not in cells stimulated with bFGF.	bind
33915	1	9364	6	10	NULL	0	NULL	cell-permeable peptide			is derived from					epidermal growth factor receptor			Grb2-binding sequence		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_18081_s_207	10364261	A cell-permeable peptide derived from the Grb2-binding sequence of epidermal growth factor receptor was shown to inhibit MAP kinase activation in cells stimulated with epidermal growth factor or with platelet-derived growth factor, but not in cells stimulated with bFGF.	bind
33916	2	9364	6	NULL	NULL	0	NULL	statement 1	NULL		inhibits	NULL				MAP kinase	NULL	activation of			NULL	cells stimulated with epidermal growth factor	0	NULL	NULL	NULL	gw60_jbiolchem_274_25_18081_s_207	10364261	A cell-permeable peptide derived from the Grb2-binding sequence of epidermal growth factor receptor was shown to inhibit MAP kinase activation in cells stimulated with epidermal growth factor or with platelet-derived growth factor, but not in cells stimulated with bFGF.	bind
33918	3	9364	6	NULL	NULL	0	NULL	statement 1	NULL		inhibits	NULL				MAP kinase	NULL	activation of			NULL	cells stimulated with platelet-derived growth factor	0	NULL	NULL	NULL	gw60_jbiolchem_274_25_18081_s_207	10364261	A cell-permeable peptide derived from the Grb2-binding sequence of epidermal growth factor receptor was shown to inhibit MAP kinase activation in cells stimulated with epidermal growth factor or with platelet-derived growth factor, but not in cells stimulated with bFGF.	bind
33919	4	9364	6	NULL	NULL	0	NULL	statement 1	NULL		does not inhibit	NULL				MAP kinase	NULL				NULL	cells stimulated with bFGF	0	NULL	NULL	NULL	gw60_jbiolchem_274_25_18081_s_207	10364261	A cell-permeable peptide derived from the Grb2-binding sequence of epidermal growth factor receptor was shown to inhibit MAP kinase activation in cells stimulated with epidermal growth factor or with platelet-derived growth factor, but not in cells stimulated with bFGF.	bind
58472	5	9364	6	10	NULL	0	NULL	statement 2			is an alternative to					statement 3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_25_18081_s_207	10364261	A cell-permeable peptide derived from the Grb2-binding sequence of epidermal growth factor receptor was shown to inhibit MAP kinase activation in cells stimulated with epidermal growth factor or with platelet-derived growth factor, but not in cells stimulated with bFGF.	bind
40743	1	9365	5	13	NULL	NULL	NULL	Shc	GP		associate with					SHP-2	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_mol-biol-cell_16_7_15888547_s_11	15888547	A cell-permeable peptide that contained a polyproline sequence  from Shc selectively inhibited Shc/SHP-2 association and impaired Shc  but not SHP-2 binding to SHPS-1.	bind
40744	2	9365	5	13	NULL	NULL	NULL	cell-permeable peptide	GP		contains					Shc	GP		polyproline sequence		NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_mol-biol-cell_16_7_15888547_s_11	15888547	A cell-permeable peptide that contained a polyproline sequence  from Shc selectively inhibited Shc/SHP-2 association and impaired Shc  but not SHP-2 binding to SHPS-1.	bind
40745	3	9365	5	13	NULL	NULL	NULL	statement 2	Process		inhibit		selectively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_mol-biol-cell_16_7_15888547_s_11	15888547	A cell-permeable peptide that contained a polyproline sequence  from Shc selectively inhibited Shc/SHP-2 association and impaired Shc  but not SHP-2 binding to SHPS-1.	bind
40746	4	9365	5	13	NULL	NULL	NULL	SHP-2	GP		bind					SHPS-1	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_mol-biol-cell_16_7_15888547_s_11	15888547	A cell-permeable peptide that contained a polyproline sequence  from Shc selectively inhibited Shc/SHP-2 association and impaired Shc  but not SHP-2 binding to SHPS-1.	bind
40747	5	9365	5	13	NULL	NULL	NULL	Shc	GP		bind					SHPS-1	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_mol-biol-cell_16_7_15888547_s_11	15888547	A cell-permeable peptide that contained a polyproline sequence  from Shc selectively inhibited Shc/SHP-2 association and impaired Shc  but not SHP-2 binding to SHPS-1.	bind
40748	6	9365	5	13	NULL	NULL	NULL	statement 2	Process		impairs					statement 5	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_mol-biol-cell_16_7_15888547_s_11	15888547	A cell-permeable peptide that contained a polyproline sequence  from Shc selectively inhibited Shc/SHP-2 association and impaired Shc  but not SHP-2 binding to SHPS-1.	bind
40749	7	9365	5	13	NULL	NULL	NULL	statement 2	Process		does not impair					statement 4	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_mol-biol-cell_16_7_15888547_s_11	15888547	A cell-permeable peptide that contained a polyproline sequence  from Shc selectively inhibited Shc/SHP-2 association and impaired Shc  but not SHP-2 binding to SHPS-1.	bind
33702	1	9365	6	NULL	NULL	0	NULL	Shc	NULL		associates with	NULL				SHP-2	NULL				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_mol-biol-cell_16_7_15888547_s_11	15888547	A cell-permeable peptide that contained a polyproline sequence  from Shc selectively inhibited Shc/SHP-2 association and impaired Shc  but not SHP-2 binding to SHPS-1.	bind
33703	2	9365	6	NULL	NULL	0	NULL	SHP-2	NULL		bind	NULL				SHPS-1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_mol-biol-cell_16_7_15888547_s_11	15888547	A cell-permeable peptide that contained a polyproline sequence  from Shc selectively inhibited Shc/SHP-2 association and impaired Shc  but not SHP-2 binding to SHPS-1.	bind
33704	3	9365	6	NULL	NULL	0	NULL	Shc	NULL		bind	NULL				SHPS-1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_mol-biol-cell_16_7_15888547_s_11	15888547	A cell-permeable peptide that contained a polyproline sequence  from Shc selectively inhibited Shc/SHP-2 association and impaired Shc  but not SHP-2 binding to SHPS-1.	bind
33705	4	9365	6	NULL	NULL	0	NULL	cell-permeable peptide	NULL		contains	NULL				Shc	NULL		polyproline sequence		NULL		0	NULL	NULL	NULL	abs-batch0517-0529_mol-biol-cell_16_7_15888547_s_11	15888547	A cell-permeable peptide that contained a polyproline sequence  from Shc selectively inhibited Shc/SHP-2 association and impaired Shc  but not SHP-2 binding to SHPS-1.	bind
33706	5	9365	6	10	NULL	0	NULL	statement 4			inhibits		selectively			statement 1					NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_mol-biol-cell_16_7_15888547_s_11	15888547	A cell-permeable peptide that contained a polyproline sequence  from Shc selectively inhibited Shc/SHP-2 association and impaired Shc  but not SHP-2 binding to SHPS-1.	bind
33759	6	9365	6	NULL	NULL	0	NULL	statement 4	NULL		inhibits	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_mol-biol-cell_16_7_15888547_s_11	15888547	A cell-permeable peptide that contained a polyproline sequence  from Shc selectively inhibited Shc/SHP-2 association and impaired Shc  but not SHP-2 binding to SHPS-1.	bind
33760	7	9365	6	NULL	NULL	0	NULL	statement 4	NULL		does not inhibit	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_mol-biol-cell_16_7_15888547_s_11	15888547	A cell-permeable peptide that contained a polyproline sequence  from Shc selectively inhibited Shc/SHP-2 association and impaired Shc  but not SHP-2 binding to SHPS-1.	bind
40750	1	9367	5	13	NULL	NULL	NULL	S-Ht31	GP		is					Ht31 counterpart	GP	cell-permeable stearated			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_4747_s_99	9030527	A cell-permeable stearated Ht31 counterpart, S-Ht31, also inhibited  in vitro binding of RII to AKAP 110, albeit at a reduced potency (85% inhibition compared with 100% by the non-stearated Ht31).	bind
40751	2	9367	5	13	NULL	NULL	NULL	RII	GP		bind					AKAP 110	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_4747_s_99	9030527	A cell-permeable stearated Ht31 counterpart, S-Ht31, also inhibited  in vitro binding of RII to AKAP 110, albeit at a reduced potency (85% inhibition compared with 100% by the non-stearated Ht31).	bind
40752	3	9367	5	13	NULL	NULL	NULL	statement 1	Process		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_4747_s_99	9030527	A cell-permeable stearated Ht31 counterpart, S-Ht31, also inhibited  in vitro binding of RII to AKAP 110, albeit at a reduced potency (85% inhibition compared with 100% by the non-stearated Ht31).	bind
40753	4	9367	5	13	NULL	NULL	NULL	Ht31	GP	non-stearated	inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_4747_s_99	9030527	A cell-permeable stearated Ht31 counterpart, S-Ht31, also inhibited  in vitro binding of RII to AKAP 110, albeit at a reduced potency (85% inhibition compared with 100% by the non-stearated Ht31).	bind
40754	5	9367	5	13	NULL	NULL	NULL	statement 3	Process	affinity of	is less than					statement 4	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_4747_s_99	9030527	A cell-permeable stearated Ht31 counterpart, S-Ht31, also inhibited  in vitro binding of RII to AKAP 110, albeit at a reduced potency (85% inhibition compared with 100% by the non-stearated Ht31).	bind
33761	1	9367	6	NULL	NULL	0	NULL	RII	NULL		bind	NULL				AKAP 110	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_272_8_4747_s_99	9030527	A cell-permeable stearated Ht31 counterpart, S-Ht31, also inhibited  in vitro binding of RII to AKAP 110, albeit at a reduced potency (85% inhibition compared with 100% by the non-stearated Ht31).	bind
33762	2	9367	6	NULL	NULL	0	NULL	S-Ht31	NULL	cell-permeable	inhibits	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_4747_s_99	9030527	A cell-permeable stearated Ht31 counterpart, S-Ht31, also inhibited  in vitro binding of RII to AKAP 110, albeit at a reduced potency (85% inhibition compared with 100% by the non-stearated Ht31).	bind
33763	3	9367	6	NULL	NULL	0	NULL	Ht31	NULL	non-stearated	inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_8_4747_s_99	9030527	A cell-permeable stearated Ht31 counterpart, S-Ht31, also inhibited  in vitro binding of RII to AKAP 110, albeit at a reduced potency (85% inhibition compared with 100% by the non-stearated Ht31).	bind
33764	4	9367	6	NULL	NULL	0	NULL	statement 2	NULL	affinity of	is less than	NULL				statement 3	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_8_4747_s_99	9030527	A cell-permeable stearated Ht31 counterpart, S-Ht31, also inhibited  in vitro binding of RII to AKAP 110, albeit at a reduced potency (85% inhibition compared with 100% by the non-stearated Ht31).	bind
33765	5	9367	6	10	NULL	0	NULL	S-Ht31			is					Ht31 counterpart		cell-permeable stearated			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_4747_s_99	9030527	A cell-permeable stearated Ht31 counterpart, S-Ht31, also inhibited  in vitro binding of RII to AKAP 110, albeit at a reduced potency (85% inhibition compared with 100% by the non-stearated Ht31).	bind
40756	1	9368	5	13	NULL	NULL	NULL	cell-permeant peptide	GP	TAT-tagged 	encompass					PAK1	GP		second proline-rich SH3 binding domain		NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
40803	2	9368	5	13	NULL	NULL	NULL	Grb2	GP		associate with					PAK1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
40804	3	9368	5	13	NULL	NULL	NULL	Grb2	GP		associate with					PAK1	GP				NULL	in vivo	NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
40805	4	9368	5	13	NULL	NULL	NULL	EGFR	GP	activated	associate with					PAK1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
40806	5	9368	5	13	NULL	NULL	NULL	EGFR	Process	activated	associate with					PAK1	Process				NULL	in vivo	NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
40807	6	9368	5	13	NULL	NULL	NULL	statement 1	Process		block					statement 2	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
40808	7	9368	5	13	NULL	NULL	NULL	statement 1	Process		block					statement 3	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
40809	8	9368	5	13	NULL	NULL	NULL	statement 1	Process		block					statement 4	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
40810	9	9368	5	13	NULL	NULL	NULL	statement 1	Process		block					statement 5	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
40811	10	9368	5	13	NULL	NULL	NULL	statement 6	Process		occurs simultaneously with					statement 8	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
40812	11	9368	5	13	NULL	NULL	NULL	statement 7	Process		occurs simultaneously with					statement 9	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
40813	12	9368	5	13	NULL	NULL	NULL	PAK1	GP		interact with					EGFR	GP	activated			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
40814	13	9368	5	13	NULL	NULL	NULL	Grb2	GP		mediate					statement 12	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
40815	14	9368	5	13	NULL	NULL	NULL	statement 10	Process		indicate					statement 13	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
40816	15	9368	5	13	NULL	NULL	NULL	statement 11	Process		indicate					statement 13	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
33920	1	9368	6	NULL	NULL	0	NULL	Grb2	NULL		associates with	NULL				PAK1	NULL				NULL	in vitro	0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
33921	2	9368	6	NULL	NULL	0	NULL	EGFR	NULL	activated	associates with	NULL				PAK1	NULL				NULL	in vivo	0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
33922	5	9368	6	10	NULL	0	NULL	Grb2	NULL		mediates	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
33923	7	9368	6	10	NULL	0	NULL	TAT-tagged peptide	NULL		encompasses	NULL				PAK1	NULL		second proline-rich SH3 binding domain		NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
49183	3	9368	6	10	NULL	0	NULL	Grb2	NULL		associates with	NULL				PAK1	NULL				NULL	in vivo	NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
49184	4	9368	6	10	NULL	0	NULL	EGFR	NULL	activated	associates with	NULL				PAK1	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
49185	6	9368	6	10	NULL	0	NULL	Grb2	NULL		mediates	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
49187	8	9368	6	10	NULL	0	NULL	statement 7	NULL		blocks	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
49188	9	9368	6	10	NULL	0	NULL	statement 7	NULL		blocks	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
49189	10	9368	6	10	NULL	0	NULL	statement 7	NULL		blocks	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
49190	11	9368	6	10	NULL	0	NULL	statement 7	NULL		blocks	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
49191	12	9368	6	10	NULL	0	NULL	statement 8	NULL		occurs simultaneously with	NULL				statement 10	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
49192	13	9368	6	10	NULL	0	NULL	statement 9	NULL		occurs simultaneously with	NULL				statement 11	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
58473	14	9368	6	10	NULL	0	NULL	statement 12			indicate					statement 5					NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
58474	15	9368	6	10	NULL	0	NULL	statement 12			indicate					statement 6					NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
58475	16	9368	6	10	NULL	0	NULL	statement 13			indicate					statement 5					NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
58476	17	9368	6	10	NULL	0	NULL	statement 13			indicate					statement 6					NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_11_12522133_s_7	12522133	A cell-permeant TAT-tagged peptide encompassing the  second proline-rich SH3 binding domain of PAK1 simultaneously blocked  Grb2 and activated EGFR association with PAK1, in vitro and in vivo, indicating  that Grb2 mediates the interaction of PAK1 with the activated EGFR.	bind
41249	1	9370	5	13	NULL	NULL	NULL	heparan sulfate proteoglycan	GP	cell-surface	mediate					neural cell	Cell	adhesion of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_1_43_s_457	7788881	A cell-surface heparan sulfate proteoglycan mediates neural cell adhesion and spreading on a defined sequence from the c-terminal cell and heparin binding domain of fibronectin, FN-C/-II.	bind
41251	2	9370	5	13	NULL	NULL	NULL	heparan sulfate proteoglycan	GP	cell-surface	mediate					neural cell	Cell	spreading of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_1_43_s_457	7788881	A cell-surface heparan sulfate proteoglycan mediates neural cell adhesion and spreading on a defined sequence from the c-terminal cell and heparin binding domain of fibronectin, FN-C/-II.	bind
33925	1	9370	6	10	NULL	0	NULL	heparan sulfate proteoglycan		cell-surface	mediates					neural cell 		adhesion of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_1_43_s_457	7788881	A cell-surface heparan sulfate proteoglycan mediates neural cell adhesion and spreading on a defined sequence from the c-terminal cell and heparin binding domain of fibronectin, FN-C/-II.	bind
33927	2	9370	6	10	NULL	0	NULL	heparan sulfate proteoglycan		cell-surface	mediates					neural cell 		spreading of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_1_43_s_457	7788881	A cell-surface heparan sulfate proteoglycan mediates neural cell adhesion and spreading on a defined sequence from the c-terminal cell and heparin binding domain of fibronectin, FN-C/-II.	bind
40817	1	9373	5	13	NULL	NULL	NULL	Zhangfei	GP		is a type of					cellular transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_clinmicrobiolrev_16_1_79_s_107	12525426	A cellular transcription factor, Zhangfei, binds to HCF and prevents activation of the ICP0 promoter ( ).	bind
40818	2	9373	5	13	NULL	NULL	NULL	Zhangfei	GP		bind					HCF	GP				NULL		NULL	NULL	NULL	NULL	gw70_clinmicrobiolrev_16_1_79_s_107	12525426	A cellular transcription factor, Zhangfei, binds to HCF and prevents activation of the ICP0 promoter ( ).	bind
40819	3	9373	5	13	NULL	NULL	NULL	statement 2	Process		prevents					ICP0	NucleicAcid	activation of		promoter	NULL		NULL	NULL	NULL	NULL	gw70_clinmicrobiolrev_16_1_79_s_107	12525426	A cellular transcription factor, Zhangfei, binds to HCF and prevents activation of the ICP0 promoter ( ).	bind
33766	1	9373	6	NULL	NULL	0	NULL	Zhangfei	NULL		is a type of	NULL				transcription factor	NULL	cellular			NULL		0	NULL	NULL	NULL	gw70_clinmicrobiolrev_16_1_79_s_107	12525426	A cellular transcription factor, Zhangfei, binds to HCF and prevents activation of the ICP0 promoter ( ).	bind
33767	2	9373	6	NULL	NULL	0	NULL	Zhangfei	NULL		bind	NULL				HCF	NULL				NULL		0	NULL	NULL	NULL	gw70_clinmicrobiolrev_16_1_79_s_107	12525426	A cellular transcription factor, Zhangfei, binds to HCF and prevents activation of the ICP0 promoter ( ).	bind
33768	3	9373	6	NULL	NULL	0	NULL	Zhangfei	NULL		prevents	NULL				ICP0	NULL	activation of		promoter	NULL		0	NULL	NULL	NULL	gw70_clinmicrobiolrev_16_1_79_s_107	12525426	A cellular transcription factor, Zhangfei, binds to HCF and prevents activation of the ICP0 promoter ( ).	bind
40820	1	9374	5	13	NULL	NULL	NULL	caveolin-1	GP		associate with								raft domains		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_161_4_673_s_17	12771123	A central dogma of the caveolae/glycolipid raft field, therefore, has been that the invaginated flask-shaped morphology of caveolae is a specific consequence of the association of caveolin-1 with select raft domains.	bind
40823	2	9374	5	13	NULL	NULL	NULL	caveolae	CellComponent		contains					flask-shaped morphology	CellComponent	invaginated			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_161_4_673_s_17	12771123	A central dogma of the caveolae/glycolipid raft field, therefore, has been that the invaginated flask-shaped morphology of caveolae is a specific consequence of the association of caveolin-1 with select raft domains.	bind
40824	3	9374	5	13	NULL	NULL	NULL	statement 2	Process		is a consequence of 					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_161_4_673_s_17	12771123	A central dogma of the caveolae/glycolipid raft field, therefore, has been that the invaginated flask-shaped morphology of caveolae is a specific consequence of the association of caveolin-1 with select raft domains.	bind
33769	1	9374	6	NULL	NULL	0	NULL	Caveolin-1	NULL		associates with	NULL					NULL		raft domains		NULL		0	NULL	NULL	NULL	gw70_cellbiol_161_4_673_s_17	12771123	A central dogma of the caveolae/glycolipid raft field, therefore, has been that the invaginated flask-shaped morphology of caveolae is a specific consequence of the association of caveolin-1 with select raft domains.	bind
33770	2	9374	6	10	NULL	0	NULL	caveolae			contains					flask-shaped morphology 		invaginated 			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_161_4_673_s_17	12771123	A central dogma of the caveolae/glycolipid raft field, therefore, has been that the invaginated flask-shaped morphology of caveolae is a specific consequence of the association of caveolin-1 with select raft domains.	bind
33771	3	9374	6	NULL	NULL	0	NULL	statement 2	NULL		is a consequence of 	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_161_4_673_s_17	12771123	A central dogma of the caveolae/glycolipid raft field, therefore, has been that the invaginated flask-shaped morphology of caveolae is a specific consequence of the association of caveolin-1 with select raft domains.	bind
40837	1	9376	5	13	NULL	NULL	NULL	Rb family	GP		regulates		negatively			E2F	GP	activities of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7455_s_12	9819431	A central function of the Rb family is to negatively regulate the activity of E2F transcription factors that control the transcription of many cell cycle-regulated genes ( 41).	bind
40838	2	9376	5	13	NULL	NULL	NULL	E2F	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7455_s_12	9819431	A central function of the Rb family is to negatively regulate the activity of E2F transcription factors that control the transcription of many cell cycle-regulated genes ( 41).	bind
40839	3	9376	5	13	NULL	NULL	NULL	E2F	GP		regulates					cell cycle-regulated genes	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7455_s_12	9819431	A central function of the Rb family is to negatively regulate the activity of E2F transcription factors that control the transcription of many cell cycle-regulated genes ( 41).	bind
33772	1	9376	6	10	NULL	0	NULL	Rb family	NULL		 regulates	NULL	negatively			E2F 	NULL	activity of 			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7455_s_12	9819431	A central function of the Rb family is to negatively regulate the activity of E2F transcription factors that control the transcription of many cell cycle-regulated genes ( 41).	bind
33773	2	9376	6	10	NULL	0	NULL	E2F 	NULL		regulate	NULL				cell cycle-regulated genes	NULL	transcription of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7455_s_12	9819431	A central function of the Rb family is to negatively regulate the activity of E2F transcription factors that control the transcription of many cell cycle-regulated genes ( 41).	bind
48124	3	9376	6	10	NULL	0	NULL	E2F	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_12_7455_s_12	9819431	A central function of the Rb family is to negatively regulate the activity of E2F transcription factors that control the transcription of many cell cycle-regulated genes ( 41).	bind
40886	1	9377	5	13	NULL	NULL	NULL	RasGAP	GP		is					Ras GTPase activating protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_17_0_701_s_436	10358772	A central protein involved in the regulation of small GTPases is the 120 kDa Ras GTPase  activating protein (RasGAP) that binds to the active, GTP-bound form of Ras and activates  its GTPase activity, catalyzing the formation of inactive Ras-GDP ( 177,  178).	bind
40887	2	9377	5	13	NULL	NULL	NULL	RasGAP	GP		is a type of					central protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_17_0_701_s_436	10358772	A central protein involved in the regulation of small GTPases is the 120 kDa Ras GTPase  activating protein (RasGAP) that binds to the active, GTP-bound form of Ras and activates  its GTPase activity, catalyzing the formation of inactive Ras-GDP ( 177,  178).	bind
40888	3	9377	5	13	NULL	NULL	NULL	RasGAP	GP		is involved in					small GTPases	GP	regulation of			NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_17_0_701_s_436	10358772	A central protein involved in the regulation of small GTPases is the 120 kDa Ras GTPase  activating protein (RasGAP) that binds to the active, GTP-bound form of Ras and activates  its GTPase activity, catalyzing the formation of inactive Ras-GDP ( 177,  178).	bind
40889	4	9377	5	13	NULL	NULL	NULL	Ras	GP		bind					GTP	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_17_0_701_s_436	10358772	A central protein involved in the regulation of small GTPases is the 120 kDa Ras GTPase  activating protein (RasGAP) that binds to the active, GTP-bound form of Ras and activates  its GTPase activity, catalyzing the formation of inactive Ras-GDP ( 177,  178).	bind
40890	5	9377	5	13	NULL	NULL	NULL	RasGAP	GP		bind					statement 4	GP	active			NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_17_0_701_s_436	10358772	A central protein involved in the regulation of small GTPases is the 120 kDa Ras GTPase  activating protein (RasGAP) that binds to the active, GTP-bound form of Ras and activates  its GTPase activity, catalyzing the formation of inactive Ras-GDP ( 177,  178).	bind
40892	7	9377	5	13	NULL	NULL	NULL	Ras-GTP	GP	active	is converted to					Ras-GDP	GP	inactive			NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_17_0_701_s_436	10358772	A central protein involved in the regulation of small GTPases is the 120 kDa Ras GTPase  activating protein (RasGAP) that binds to the active, GTP-bound form of Ras and activates  its GTPase activity, catalyzing the formation of inactive Ras-GDP ( 177,  178).	bind
40893	8	9377	5	13	NULL	NULL	NULL	statement 6	Process		catalyze					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_17_0_701_s_436	10358772	A central protein involved in the regulation of small GTPases is the 120 kDa Ras GTPase  activating protein (RasGAP) that binds to the active, GTP-bound form of Ras and activates  its GTPase activity, catalyzing the formation of inactive Ras-GDP ( 177,  178).	bind
48125	6	9377	5	13	NULL	NULL	NULL	statement 5	Process		activates					Ras	GP	GTPase activity of			NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_17_0_701_s_436	10358772	A central protein involved in the regulation of small GTPases is the 120 kDa Ras GTPase  activating protein (RasGAP) that binds to the active, GTP-bound form of Ras and activates  its GTPase activity, catalyzing the formation of inactive Ras-GDP ( 177,  178).	bind
33774	1	9377	6	NULL	NULL	0	NULL	RasGAP	NULL		is	NULL				Ras GTPase activating protein	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_701_s_436	10358772	A central protein involved in the regulation of small GTPases is the 120 kDa Ras GTPase  activating protein (RasGAP) that binds to the active, GTP-bound form of Ras and activates  its GTPase activity, catalyzing the formation of inactive Ras-GDP ( 177,  178).	bind
33775	2	9377	6	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				Ras	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_701_s_436	10358772	A central protein involved in the regulation of small GTPases is the 120 kDa Ras GTPase  activating protein (RasGAP) that binds to the active, GTP-bound form of Ras and activates  its GTPase activity, catalyzing the formation of inactive Ras-GDP ( 177,  178).	bind
33776	3	9377	6	NULL	NULL	0	NULL	RasGAP	NULL		bind	NULL				statement 2	NULL	active			NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_701_s_436	10358772	A central protein involved in the regulation of small GTPases is the 120 kDa Ras GTPase  activating protein (RasGAP) that binds to the active, GTP-bound form of Ras and activates  its GTPase activity, catalyzing the formation of inactive Ras-GDP ( 177,  178).	bind
33777	4	9377	6	10	NULL	0	NULL	statement 2			activates					Ras		GTPase activity of			NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_17_0_701_s_436	10358772	A central protein involved in the regulation of small GTPases is the 120 kDa Ras GTPase  activating protein (RasGAP) that binds to the active, GTP-bound form of Ras and activates  its GTPase activity, catalyzing the formation of inactive Ras-GDP ( 177,  178).	bind
33779	7	9377	6	10	NULL	0	NULL	statement 4	NULL		catalyzes	NULL				statement 6	NULL				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_17_0_701_s_436	10358772	A central protein involved in the regulation of small GTPases is the 120 kDa Ras GTPase  activating protein (RasGAP) that binds to the active, GTP-bound form of Ras and activates  its GTPase activity, catalyzing the formation of inactive Ras-GDP ( 177,  178).	bind
48126	6	9377	6	10	NULL	0	NULL	RAS-GTP	NULL	active	is converted to	NULL				RAS-GDP	NULL	inactive			NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_701_s_436	10358772	A central protein involved in the regulation of small GTPases is the 120 kDa Ras GTPase  activating protein (RasGAP) that binds to the active, GTP-bound form of Ras and activates  its GTPase activity, catalyzing the formation of inactive Ras-GDP ( 177,  178).	bind
58477	5	9377	6	10	NULL	0	NULL	RasGAP			is involved in					small GTPases		regulation of			NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_701_s_436	10358772	A central protein involved in the regulation of small GTPases is the 120 kDa Ras GTPase  activating protein (RasGAP) that binds to the active, GTP-bound form of Ras and activates  its GTPase activity, catalyzing the formation of inactive Ras-GDP ( 177,  178).	bind
40894	1	9378	5	13	NULL	NULL	NULL	PSGL-1	GP		bind					E-selectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_45_28786_s_161	9353350	A central question arising from the current study is how the E-selectin and the P-selectin binding activities of PSGL-1 could be differentially regulated and what the structural differences between both recognition motifs are.	bind
40895	2	9378	5	13	NULL	NULL	NULL	PSGL-1	GP		bind					P-selectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_45_28786_s_161	9353350	A central question arising from the current study is how the E-selectin and the P-selectin binding activities of PSGL-1 could be differentially regulated and what the structural differences between both recognition motifs are.	bind
33780	1	9378	6	NULL	NULL	0	NULL	PSGL-1	NULL		bind	NULL				E-selectin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_45_28786_s_161	9353350	A central question arising from the current study is how the E-selectin and the P-selectin binding activities of PSGL-1 could be differentially regulated and what the structural differences between both recognition motifs are.	bind
33781	2	9378	6	NULL	NULL	0	NULL	PSGL-1	NULL		bind	NULL				P-selectin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_45_28786_s_161	9353350	A central question arising from the current study is how the E-selectin and the P-selectin binding activities of PSGL-1 could be differentially regulated and what the structural differences between both recognition motifs are.	bind
40896	1	9379	5	13	NULL	NULL	NULL	rhodopsin	GP	MII form of 	bind					transducin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_3_1683_s_17	9880548	A central question remains as to why only the MII form of rhodopsin can bind and activate transducin.	bind
40897	2	9379	5	13	NULL	NULL	NULL	statement 1	Process		activates					transducin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_3_1683_s_17	9880548	A central question remains as to why only the MII form of rhodopsin can bind and activate transducin.	bind
33782	1	9379	6	NULL	NULL	0	NULL	rhodopsin	NULL	MII form	bind	NULL				transducin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_3_1683_s_17	9880548	A central question remains as to why only the MII form of rhodopsin can bind and activate transducin.	bind
33783	2	9379	6	NULL	NULL	0	NULL	rhodopsin	NULL	MII form	activates	NULL				transducin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_3_1683_s_17	9880548	A central question remains as to why only the MII form of rhodopsin can bind and activate transducin.	bind
41234	1	9380	5	13	NULL	NULL	NULL	mTERF	GP		is					mitochondrial transcription termination factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_15_15670_s_18	14744862	A central role in the attenuation phenomenon taking place at this site is played by the mitochondrial transcription termination factor (mTERF),  1 a 39-kDa DNA-binding protein that binds to a 28-base pair region (nucleotides 3229 to 3256) within the  tRNALeu(UUR) gene, at a position immediately adjacent to the  16 S rRNA gene.	bind
41237	2	9380	5	13	NULL	NULL	NULL	mTERF	GP		is a type of					DNA-binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_15_15670_s_18	14744862	A central role in the attenuation phenomenon taking place at this site is played by the mitochondrial transcription termination factor (mTERF),  1 a 39-kDa DNA-binding protein that binds to a 28-base pair region (nucleotides 3229 to 3256) within the  tRNALeu(UUR) gene, at a position immediately adjacent to the  16 S rRNA gene.	bind
41238	3	9380	5	13	NULL	NULL	NULL	mTERF	GP		bind					tRNALeu(UUR) gene	GP			28-base pair region (nucleotides 3229 to 3256)	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_15_15670_s_18	14744862	A central role in the attenuation phenomenon taking place at this site is played by the mitochondrial transcription termination factor (mTERF),  1 a 39-kDa DNA-binding protein that binds to a 28-base pair region (nucleotides 3229 to 3256) within the  tRNALeu(UUR) gene, at a position immediately adjacent to the  16 S rRNA gene.	bind
41242	4	9380	5	13	NULL	NULL	NULL	statement 3	Process		occurs					16 S rRNA gene	GP	adjacent to			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_15_15670_s_18	14744862	A central role in the attenuation phenomenon taking place at this site is played by the mitochondrial transcription termination factor (mTERF),  1 a 39-kDa DNA-binding protein that binds to a 28-base pair region (nucleotides 3229 to 3256) within the  tRNALeu(UUR) gene, at a position immediately adjacent to the  16 S rRNA gene.	bind
33784	1	9380	6	NULL	NULL	0	NULL	mTERF	NULL		is	NULL				mitochondrial transcription termination factor	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_15_15670_s_18	14744862	A central role in the attenuation phenomenon taking place at this site is played by the mitochondrial transcription termination factor (mTERF),  1 a 39-kDa DNA-binding protein that binds to a 28-base pair region (nucleotides 3229 to 3256) within the  tRNALeu(UUR) gene, at a position immediately adjacent to the  16 S rRNA gene.	bind
33930	2	9380	6	10	NULL	0	NULL	mTERF			bind					tRNALeu(UUR) gene				28-base pair region nucleotides 3229 to 3256	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_15_15670_s_18	14744862	A central role in the attenuation phenomenon taking place at this site is played by the mitochondrial transcription termination factor (mTERF),  1 a 39-kDa DNA-binding protein that binds to a 28-base pair region (nucleotides 3229 to 3256) within the  tRNALeu(UUR) gene, at a position immediately adjacent to the  16 S rRNA gene.	bind
33932	3	9380	6	10	NULL	0	NULL	mTERF	NULL		is a type of	NULL				DNA-binding protein	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_15_15670_s_18	14744862	A central role in the attenuation phenomenon taking place at this site is played by the mitochondrial transcription termination factor (mTERF),  1 a 39-kDa DNA-binding protein that binds to a 28-base pair region (nucleotides 3229 to 3256) within the  tRNALeu(UUR) gene, at a position immediately adjacent to the  16 S rRNA gene.	bind
48127	4	9380	6	10	NULL	0	NULL	statement 2	NULL		occurs	NULL				16 S rRNA gene	NULL	adjacent to			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_15_15670_s_18	14744862	A central role in the attenuation phenomenon taking place at this site is played by the mitochondrial transcription termination factor (mTERF),  1 a 39-kDa DNA-binding protein that binds to a 28-base pair region (nucleotides 3229 to 3256) within the  tRNALeu(UUR) gene, at a position immediately adjacent to the  16 S rRNA gene.	bind
40898	1	9381	5	13	NULL	NULL	NULL	CREB	GP		bind		constitutively							CRE	NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_37_13572_s_6	15342915	A central tenet of the CREB - CBP model is that CREB binds constitutively to the CRE and that regulation occurs through the phosphorylation-dependent recruitment of CBP.	bind
40899	2	9381	5	13	NULL	NULL	NULL	CBP	GP	recruitment of	is dependent on					phosphorylation	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_37_13572_s_6	15342915	A central tenet of the CREB - CBP model is that CREB binds constitutively to the CRE and that regulation occurs through the phosphorylation-dependent recruitment of CBP.	bind
40900	3	9381	5	13	NULL	NULL	NULL	statement 1	Process	regulation of	occurs through					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_37_13572_s_6	15342915	A central tenet of the CREB - CBP model is that CREB binds constitutively to the CRE and that regulation occurs through the phosphorylation-dependent recruitment of CBP.	bind
33785	1	9381	6	10	NULL	0	NULL	CREB			bind 		constitutively							CRE	NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_37_13572_s_6	15342915	A central tenet of the CREB - CBP model is that CREB binds constitutively to the CRE and that regulation occurs through the phosphorylation-dependent recruitment of CBP.	bind
33786	2	9381	6	NULL	NULL	0	NULL	CBP	NULL	recruitment of	is dependent on	NULL				phosphorylation	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_101_37_13572_s_6	15342915	A central tenet of the CREB - CBP model is that CREB binds constitutively to the CRE and that regulation occurs through the phosphorylation-dependent recruitment of CBP.	bind
33787	3	9381	6	10	NULL	0	NULL	statement 1	NULL	regulation of	occurs through	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_37_13572_s_6	15342915	A central tenet of the CREB - CBP model is that CREB binds constitutively to the CRE and that regulation occurs through the phosphorylation-dependent recruitment of CBP.	bind
40901	1	9382	5	13	NULL	NULL	NULL	cortactin	GP		constitutes					series of repeats	GP	centrally positioned			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_162_1_99_s_40	12835311	A centrally positioned series of repeats in cortactin bind and cross-link actin filaments in a tyrosine phosphorylation - dependent manner ( ;  ).	bind
40902	2	9382	5	13	NULL	NULL	NULL	statement 1	GP		bind					actin filaments	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_162_1_99_s_40	12835311	A centrally positioned series of repeats in cortactin bind and cross-link actin filaments in a tyrosine phosphorylation - dependent manner ( ;  ).	bind
40903	3	9382	5	13	NULL	NULL	NULL	statement 1	GP		cross-links					actin filaments	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_162_1_99_s_40	12835311	A centrally positioned series of repeats in cortactin bind and cross-link actin filaments in a tyrosine phosphorylation - dependent manner ( ;  ).	bind
40904	4	9382	5	13	NULL	NULL	NULL	statement 2	Process		is dependent on					phosphorylation	Process		tyrosine		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_162_1_99_s_40	12835311	A centrally positioned series of repeats in cortactin bind and cross-link actin filaments in a tyrosine phosphorylation - dependent manner ( ;  ).	bind
40905	5	9382	5	13	NULL	NULL	NULL	statement 3	Process		is dependent on					phosphorylation	Process		tyrosine		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_162_1_99_s_40	12835311	A centrally positioned series of repeats in cortactin bind and cross-link actin filaments in a tyrosine phosphorylation - dependent manner ( ;  ).	bind
33788	1	9382	6	NULL	NULL	0	NULL	cortactin	NULL		bind	NULL		centrally positioned series of repeats		actin filaments	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_162_1_99_s_40	12835311	A centrally positioned series of repeats in cortactin bind and cross-link actin filaments in a tyrosine phosphorylation - dependent manner ( ;  ).	bind
33789	2	9382	6	NULL	NULL	0	NULL	cortactin	NULL		cross link	NULL		centrally positioned series of repeats		actin filaments	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_162_1_99_s_40	12835311	A centrally positioned series of repeats in cortactin bind and cross-link actin filaments in a tyrosine phosphorylation - dependent manner ( ;  ).	bind
33790	3	9382	6	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				tyrosine	NULL	phosphorylation of			NULL		0	NULL	NULL	NULL	gw70_cellbiol_162_1_99_s_40	12835311	A centrally positioned series of repeats in cortactin bind and cross-link actin filaments in a tyrosine phosphorylation - dependent manner ( ;  ).	bind
33791	4	9382	6	NULL	NULL	0	NULL	statement 2	NULL		is dependent on	NULL				tyrosine	NULL	phosphorylation of			NULL		0	NULL	NULL	NULL	gw70_cellbiol_162_1_99_s_40	12835311	A centrally positioned series of repeats in cortactin bind and cross-link actin filaments in a tyrosine phosphorylation - dependent manner ( ;  ).	bind
40906	1	9383	5	13	NULL	NULL	NULL	TIMP-2	GP		bind					MT1-MMP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_38_24360_s_266	9733724	A certain amount of TIMP-2 bound to MT1-MMP appears to be required for efficient activation of pro-MMP-2.	bind
40907	2	9383	5	13	NULL	NULL	NULL	statement 1	Process		is required for					pro-MMP-2	GP	efficient activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_38_24360_s_266	9733724	A certain amount of TIMP-2 bound to MT1-MMP appears to be required for efficient activation of pro-MMP-2.	bind
33792	1	9383	6	NULL	NULL	0	NULL	TIMP-2	NULL		bind	NULL				MT1-MMP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_38_24360_s_266	9733724	A certain amount of TIMP-2 bound to MT1-MMP appears to be required for efficient activation of pro-MMP-2.	bind
33793	2	9383	6	NULL	NULL	0	NULL	statement 1	NULL		is required for	NULL				pro-MMP-2	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_38_24360_s_266	9733724	A certain amount of TIMP-2 bound to MT1-MMP appears to be required for efficient activation of pro-MMP-2.	bind
40908	1	9384	5	13	NULL	NULL	NULL	p85	GP		bind					Grb2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_26_16670_s_224	9195983	A certain conclusion is that binding of p85 and p120 to Grb2 occurs independently: while the binding of p85 is lost if only the C-SH3 domain is intact, this alteration does not affect the association of p120.	bind
40909	2	9384	5	13	NULL	NULL	NULL	p120	GP		bind					Grb2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_26_16670_s_224	9195983	A certain conclusion is that binding of p85 and p120 to Grb2 occurs independently: while the binding of p85 is lost if only the C-SH3 domain is intact, this alteration does not affect the association of p120.	bind
40910	3	9384	5	13	NULL	NULL	NULL	statement 1	Process		is independent of					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_26_16670_s_224	9195983	A certain conclusion is that binding of p85 and p120 to Grb2 occurs independently: while the binding of p85 is lost if only the C-SH3 domain is intact, this alteration does not affect the association of p120.	bind
40927	4	9384	5	13	NULL	NULL	NULL				disrupt			intact C-SH3 domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_26_16670_s_224	9195983	A certain conclusion is that binding of p85 and p120 to Grb2 occurs independently: while the binding of p85 is lost if only the C-SH3 domain is intact, this alteration does not affect the association of p120.	bind
40928	5	9384	5	13	NULL	NULL	NULL				does not affect			intact C-SH3 domain		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_26_16670_s_224	9195983	A certain conclusion is that binding of p85 and p120 to Grb2 occurs independently: while the binding of p85 is lost if only the C-SH3 domain is intact, this alteration does not affect the association of p120.	bind
33794	1	9384	6	NULL	NULL	0	NULL	p85	NULL		bind	NULL				Grb2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_26_16670_s_224	9195983	A certain conclusion is that binding of p85 and p120 to Grb2 occurs independently: while the binding of p85 is lost if only the C-SH3 domain is intact, this alteration does not affect the association of p120.	bind
33795	2	9384	6	NULL	NULL	0	NULL	p120	NULL		bind	NULL				Grb2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_26_16670_s_224	9195983	A certain conclusion is that binding of p85 and p120 to Grb2 occurs independently: while the binding of p85 is lost if only the C-SH3 domain is intact, this alteration does not affect the association of p120.	bind
33796	3	9384	6	NULL	NULL	0	NULL	statement 1	NULL		is independent of	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_26_16670_s_224	9195983	A certain conclusion is that binding of p85 and p120 to Grb2 occurs independently: while the binding of p85 is lost if only the C-SH3 domain is intact, this alteration does not affect the association of p120.	bind
33797	4	9384	6	10	NULL	0	NULL	p85	NULL	binding of	is lost 	NULL					NULL	in presence of;;intact	C-SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_26_16670_s_224	9195983	A certain conclusion is that binding of p85 and p120 to Grb2 occurs independently: while the binding of p85 is lost if only the C-SH3 domain is intact, this alteration does not affect the association of p120.	bind
33798	5	9384	6	10	NULL	0	NULL	p120	NULL	binding of	has no effect of	NULL					NULL	in presence of	C-SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_26_16670_s_224	9195983	A certain conclusion is that binding of p85 and p120 to Grb2 occurs independently: while the binding of p85 is lost if only the C-SH3 domain is intact, this alteration does not affect the association of p120.	bind
40931	2	9385	5	13	NULL	NULL	NULL	statement 1	GP		bind					AP-2 complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3655_s_89	10652362	A CFTR-derived Fusion Protein Binds to the AP-2 Complex but Not the AP-1 Complex-- The role of the carboxyl terminus of CFTR as a site for AP-2 interaction was evaluated further by generating a GST fusion protein corresponding to amino acids 1404-1480.	bind
40932	3	9385	5	13	NULL	NULL	NULL	statement 1	GP		does not bind					AP-1 complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3655_s_89	10652362	A CFTR-derived Fusion Protein Binds to the AP-2 Complex but Not the AP-1 Complex-- The role of the carboxyl terminus of CFTR as a site for AP-2 interaction was evaluated further by generating a GST fusion protein corresponding to amino acids 1404-1480.	bind
48128	1	9385	5	13	NULL	NULL	NULL	Fusion Protein	GP		derived from					CFTR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3655_s_89	10652362	A CFTR-derived Fusion Protein Binds to the AP-2 Complex but Not the AP-1 Complex-- The role of the carboxyl terminus of CFTR as a site for AP-2 interaction was evaluated further by generating a GST fusion protein corresponding to amino acids 1404-1480.	bind
33837	2	9385	6	10	NULL	0	NULL	statement 1	NULL		bind	NULL				AP-2 complex	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3655_s_89	10652362	A CFTR-derived Fusion Protein Binds to the AP-2 Complex but Not the AP-1 Complex-- The role of the carboxyl terminus of CFTR as a site for AP-2 interaction was evaluated further by generating a GST fusion protein corresponding to amino acids 1404-1480.	bind
33838	3	9385	6	10	NULL	0	NULL	statement 1	NULL		does not bind	NULL				AP-1 complex	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3655_s_89	10652362	A CFTR-derived Fusion Protein Binds to the AP-2 Complex but Not the AP-1 Complex-- The role of the carboxyl terminus of CFTR as a site for AP-2 interaction was evaluated further by generating a GST fusion protein corresponding to amino acids 1404-1480.	bind
48129	1	9385	6	10	NULL	0	NULL	fusion protein	NULL		derived from	NULL				CFTR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_5_3655_s_89	10652362	A CFTR-derived Fusion Protein Binds to the AP-2 Complex but Not the AP-1 Complex-- The role of the carboxyl terminus of CFTR as a site for AP-2 interaction was evaluated further by generating a GST fusion protein corresponding to amino acids 1404-1480.	bind
40937	1	9388	5	13	NULL	NULL	NULL				bind			polyproline type II helix		Hck	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_48_32129_s_194	9822689	A change in accessibility of the SH3 domain is not surprising, given the proximity of Trp260 to the polyproline type II helix that is bound by the SH3 domain of Hck.	bind
33839	1	9388	6	NULL	NULL	0	NULL	Hck	NULL		bind	NULL		SH3 domain			NULL		polyproline type II helix		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_48_32129_s_194	9822689	A change in accessibility of the SH3 domain is not surprising, given the proximity of Trp260 to the polyproline type II helix that is bound by the SH3 domain of Hck.	bind
40938	1	9389	5	13	NULL	NULL	NULL	apolipoprotein E	GP		bind					very low density lipoprotein	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3542_s_628	9437204	A change in apolipoprotein B expression is required for the binding of apolipoprotein E to very low density lipoprotein.	bind
40939	2	9389	5	13	NULL	NULL	NULL	apolipoprotein B	GP	change in expression of	is required for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3542_s_628	9437204	A change in apolipoprotein B expression is required for the binding of apolipoprotein E to very low density lipoprotein.	bind
33840	1	9389	6	NULL	NULL	0	NULL	apolipoprotein E	NULL		bind	NULL				very low density lipoprotein	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3542_s_628	9437204	A change in apolipoprotein B expression is required for the binding of apolipoprotein E to very low density lipoprotein.	bind
33841	2	9389	6	10	NULL	0	NULL	statement 1	NULL		is required for 	NULL				apolipoprotein B 	NULL	change in expression of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_12_3542_s_628	9437204	A change in apolipoprotein B expression is required for the binding of apolipoprotein E to very low density lipoprotein.	bind
41027	1	9390	5	13	NULL	NULL	NULL	PO4 group	Chemical	negatively charged	is a constituent of					CPP ligand	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainres_891_1_266_s_151	11164831	A change in charge of the receptor may allow for increased binding of the negatively charged PO4 group of the CPP ligand, the critical structural component for CPP binding [  12].	bind
41028	2	9390	5	13	NULL	NULL	NULL	receptor	GP	change in charge of	increase		may			statement 1	Process	 binding of			NULL		NULL	NULL	NULL	NULL	gw60_brainres_891_1_266_s_151	11164831	A change in charge of the receptor may allow for increased binding of the negatively charged PO4 group of the CPP ligand, the critical structural component for CPP binding [  12].	bind
41029	3	9390	5	13	NULL	NULL	NULL	CPP ligand	GP	negatively charged	is critical for			PO4 group		CPP	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_brainres_891_1_266_s_151	11164831	A change in charge of the receptor may allow for increased binding of the negatively charged PO4 group of the CPP ligand, the critical structural component for CPP binding [  12].	bind
33842	1	9390	6	10	NULL	0	NULL	PO4 group	NULL	negatively charged	is a constituent of	NULL				CPP ligand	NULL				NULL		NULL	NULL	NULL	NULL	gw60_brainres_891_1_266_s_151	11164831	A change in charge of the receptor may allow for increased binding of the negatively charged PO4 group of the CPP ligand, the critical structural component for CPP binding [  12].	bind
34055	2	9390	6	10	NULL	0	NULL	CPP ligand	NULL	 negatively charged	is critical for	NULL		PO4 group		CPP	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw60_brainres_891_1_266_s_151	11164831	A change in charge of the receptor may allow for increased binding of the negatively charged PO4 group of the CPP ligand, the critical structural component for CPP binding [  12].	bind
34056	3	9390	6	10	NULL	0	NULL	receptor	NULL	change in charge of	increase	NULL	may			statement 1	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw60_brainres_891_1_266_s_151	11164831	A change in charge of the receptor may allow for increased binding of the negatively charged PO4 group of the CPP ligand, the critical structural component for CPP binding [  12].	bind
40950	1	9391	5	13	NULL	NULL	NULL	Cu2+	Chemical		bind					Abeta	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_5_2977_s_170	12435742	A change in the coordination mode of the Cu2+ bound to Abeta at higher pH that also reduces the oligomerization of the peptides would explain the observed reduction of copper-induced MLRC by Abeta40 at these pH values.	bind
40951	3	9391	5	13	NULL	NULL	NULL	statement 1	Process		occurs at					high pH	QuantityOrMeasure				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_5_2977_s_170	12435742	A change in the coordination mode of the Cu2+ bound to Abeta at higher pH that also reduces the oligomerization of the peptides would explain the observed reduction of copper-induced MLRC by Abeta40 at these pH values.	bind
40952	2	9391	5	13	NULL	NULL	NULL	statement 1	Process		reduce					peptides	GP	oligomerization of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_5_2977_s_170	12435742	A change in the coordination mode of the Cu2+ bound to Abeta at higher pH that also reduces the oligomerization of the peptides would explain the observed reduction of copper-induced MLRC by Abeta40 at these pH values.	bind
41013	4	9391	5	13	NULL	NULL	NULL	copper	Chemical		induce					MLRC	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_5_2977_s_170	12435742	A change in the coordination mode of the Cu2+ bound to Abeta at higher pH that also reduces the oligomerization of the peptides would explain the observed reduction of copper-induced MLRC by Abeta40 at these pH values.	bind
41014	5	9391	5	13	NULL	NULL	NULL	Abeta40	GP		reduce					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_5_2977_s_170	12435742	A change in the coordination mode of the Cu2+ bound to Abeta at higher pH that also reduces the oligomerization of the peptides would explain the observed reduction of copper-induced MLRC by Abeta40 at these pH values.	bind
41016	6	9391	5	13	NULL	NULL	NULL	statement 2	Process		explains					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_5_2977_s_170	12435742	A change in the coordination mode of the Cu2+ bound to Abeta at higher pH that also reduces the oligomerization of the peptides would explain the observed reduction of copper-induced MLRC by Abeta40 at these pH values.	bind
33843	1	9391	6	NULL	NULL	0	NULL	Cu2+	NULL		bind	NULL				Abeta	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_5_2977_s_170	12435742	A change in the coordination mode of the Cu2+ bound to Abeta at higher pH that also reduces the oligomerization of the peptides would explain the observed reduction of copper-induced MLRC by Abeta40 at these pH values.	bind
33934	3	9391	6	10	NULL	0	NULL	Abeta40	NULL		reduces	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_5_2977_s_170	12435742	A change in the coordination mode of the Cu2+ bound to Abeta at higher pH that also reduces the oligomerization of the peptides would explain the observed reduction of copper-induced MLRC by Abeta40 at these pH values.	bind
48130	2	9391	6	10	NULL	0	NULL	copper	NULL		induce	NULL				MLRC	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_5_2977_s_170	12435742	A change in the coordination mode of the Cu2+ bound to Abeta at higher pH that also reduces the oligomerization of the peptides would explain the observed reduction of copper-induced MLRC by Abeta40 at these pH values.	bind
48131	4	9391	6	10	NULL	0	NULL	statement 1	NULL		reduce	NULL				peptides	NULL	oligomerization of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_5_2977_s_170	12435742	A change in the coordination mode of the Cu2+ bound to Abeta at higher pH that also reduces the oligomerization of the peptides would explain the observed reduction of copper-induced MLRC by Abeta40 at these pH values.	bind
48132	5	9391	6	10	NULL	0	NULL	statement 1	NULL		occurs at	NULL				high pH	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_5_2977_s_170	12435742	A change in the coordination mode of the Cu2+ bound to Abeta at higher pH that also reduces the oligomerization of the peptides would explain the observed reduction of copper-induced MLRC by Abeta40 at these pH values.	bind
58478	6	9391	6	10	NULL	0	NULL	statement 4			explains					statement 3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_5_2977_s_170	12435742	A change in the coordination mode of the Cu2+ bound to Abeta at higher pH that also reduces the oligomerization of the peptides would explain the observed reduction of copper-induced MLRC by Abeta40 at these pH values.	bind
41017	1	9392	5	13	NULL	NULL	NULL	HIV-1 capsid	CellComponent	change in	decrease			cyclophilin A-binding loop		TRIM5alpha	GP	binding of;;human	R332P		NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-virol_80_14_16809279_s_6	16809279	A change in the cyclophilin A-binding loop of the HIV-1 capsid  decreased TRIM5alpha(hu) R332P binding and allowed escape from restriction.	bind
41018	2	9392	5	13	NULL	NULL	NULL	statement 1	Process		allows					restriction	Process	escape from			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-virol_80_14_16809279_s_6	16809279	A change in the cyclophilin A-binding loop of the HIV-1 capsid  decreased TRIM5alpha(hu) R332P binding and allowed escape from restriction.	bind
33937	1	9392	6	10	NULL	0	NULL	HIV-1 capsid		change in	decreases			cyclophilin A-binding loop		TRIM5alpha(hu) 		binding of	R332P		NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-virol_80_14_16809279_s_6	16809279	A change in the cyclophilin A-binding loop of the HIV-1 capsid  decreased TRIM5alpha(hu) R332P binding and allowed escape from restriction.	bind
58479	2	9392	6	10	NULL	0	NULL	statement 1			allows					restriction		escape from			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-virol_80_14_16809279_s_6	16809279	A change in the cyclophilin A-binding loop of the HIV-1 capsid  decreased TRIM5alpha(hu) R332P binding and allowed escape from restriction.	bind
41019	1	9393	5	13	NULL	NULL	NULL	FLP	GP		is changed to			arginine at position 191		FLP	GP		lysine		NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-mol-biol_225_2_1593623_s_6	1593623	A change of arginine at position  191 to lysine resulted in a protein (FLP-R191K) that could bind to the  FRT site but could not catalyze recombination.	bind
41020	2	9393	5	13	NULL	NULL	NULL	statement 1	Process		results in					FLP	GP		R191K		NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-mol-biol_225_2_1593623_s_6	1593623	A change of arginine at position  191 to lysine resulted in a protein (FLP-R191K) that could bind to the  FRT site but could not catalyze recombination.	bind
41021	3	9393	5	13	NULL	NULL	NULL	FLP	GP		bind			R191K						FRT site	NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-mol-biol_225_2_1593623_s_6	1593623	A change of arginine at position  191 to lysine resulted in a protein (FLP-R191K) that could bind to the  FRT site but could not catalyze recombination.	bind
41022	4	9393	5	13	NULL	NULL	NULL	FLP	GP		does not catalyze			R191K		recombination					NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-mol-biol_225_2_1593623_s_6	1593623	A change of arginine at position  191 to lysine resulted in a protein (FLP-R191K) that could bind to the  FRT site but could not catalyze recombination.	bind
33844	1	9393	6	10	NULL	0	NULL	FLP			is changed to			arginine at position 191		FLP			Lysine at position 191		NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-mol-biol_225_2_1593623_s_6	1593623	A change of arginine at position  191 to lysine resulted in a protein (FLP-R191K) that could bind to the  FRT site but could not catalyze recombination.	bind
33845	2	9393	6	NULL	NULL	0	NULL	statement 1	NULL		results in	NULL				FLP	NULL		R191K		NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-mol-biol_225_2_1593623_s_6	1593623	A change of arginine at position  191 to lysine resulted in a protein (FLP-R191K) that could bind to the  FRT site but could not catalyze recombination.	bind
33846	3	9393	6	NULL	NULL	0	NULL	FLP	NULL		bind	NULL		R191K			NULL			FRT site	NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-mol-biol_225_2_1593623_s_6	1593623	A change of arginine at position  191 to lysine resulted in a protein (FLP-R191K) that could bind to the  FRT site but could not catalyze recombination.	bind
33847	4	9393	6	10	NULL	0	NULL	FLP	NULL		does not catalyze	NULL		R191K		recombination	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-mol-biol_225_2_1593623_s_6	1593623	A change of arginine at position  191 to lysine resulted in a protein (FLP-R191K) that could bind to the  FRT site but could not catalyze recombination.	bind
41023	1	9394	5	13	NULL	NULL	NULL	channel/pore-like protein	GP		allows					plus-or-minus 107 molecules s 1	GP	transport of			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1613_1_57_s_330	12832087	A channel/pore-like protein should allow transport of  plus-or-minus 107 molecules s 1, while permeases allowing equilibrating facilitated diffusion characterised so far,  allow transport with  Vmax 105 molecules s 1 [  44] and active transporters generally present lower  Vmax, 10-103 molecules s 1 [ 44].	bind
41024	2	9394	5	13	NULL	NULL	NULL	permeases	GP		allows					facilitated diffusion	Process	equilibrating 			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1613_1_57_s_330	12832087	A channel/pore-like protein should allow transport of  plus-or-minus 107 molecules s 1, while permeases allowing equilibrating facilitated diffusion characterised so far,  allow transport with  Vmax 105 molecules s 1 [  44] and active transporters generally present lower  Vmax, 10-103 molecules s 1 [ 44].	bind
33942	1	9394	6	NULL	NULL	0	NULL	channel/pore-like protein	NULL		allows	NULL				plus-or-minus 107 molecules	NULL	transport of 			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1613_1_57_s_330	12832087	A channel/pore-like protein should allow transport of  plus-or-minus 107 molecules s 1, while permeases allowing equilibrating facilitated diffusion characterised so far,  allow transport with  Vmax 105 molecules s 1 [  44] and active transporters generally present lower  Vmax, 10-103 molecules s 1 [ 44].	bind
33943	2	9394	6	NULL	NULL	0	NULL	permeases	NULL		equilibrate	NULL				facilitated diffusion	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1613_1_57_s_330	12832087	A channel/pore-like protein should allow transport of  plus-or-minus 107 molecules s 1, while permeases allowing equilibrating facilitated diffusion characterised so far,  allow transport with  Vmax 105 molecules s 1 [  44] and active transporters generally present lower  Vmax, 10-103 molecules s 1 [ 44].	bind
41030	1	9395	5	13	NULL	NULL	NULL	ETS domain	GP		is a type of					85-amino-acid-long DNA-binding motif	GP	highly conserved			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7300_s_13	10982847	A characteristic feature of this class of proteins is a highly conserved, 85-amino-acid-long DNA-binding motif termed the ETS domain, which specifically binds to GGA(A/T)-containing DNA target sequences.	bind
41031	2	9395	5	13	NULL	NULL	NULL				bind		specifically	ETS domain		DNA target sequences	NucleicAcid			GGA(A/T)	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7300_s_13	10982847	A characteristic feature of this class of proteins is a highly conserved, 85-amino-acid-long DNA-binding motif termed the ETS domain, which specifically binds to GGA(A/T)-containing DNA target sequences.	bind
33848	1	9395	6	10	NULL	0	NULL		NULL		bind	NULL	specifically	ETS domain		DNA target sequences	NULL			GGA(A/T)-containing 	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7300_s_13	10982847	A characteristic feature of this class of proteins is a highly conserved, 85-amino-acid-long DNA-binding motif termed the ETS domain, which specifically binds to GGA(A/T)-containing DNA target sequences.	bind
48133	2	9395	6	10	NULL	0	NULL	ETS domain	NULL		is a type of	NULL				85-amino-acid-long DNA-binding motif 	NULL	highly conserved			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7300_s_13	10982847	A characteristic feature of this class of proteins is a highly conserved, 85-amino-acid-long DNA-binding motif termed the ETS domain, which specifically binds to GGA(A/T)-containing DNA target sequences.	bind
41032	1	9396	5	13	NULL	NULL	NULL	adhesins	GP	bacterial	bind					extracellular matrix proteins	GP	eukaryotic			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_17_5842_s_290	15317790	A characteristic of bacterial adhesins that bind to eukaryotic extracellular matrix proteins is the presence of amino acid repeats ( ).	bind
41033	2	9396	5	13	NULL	NULL	NULL			presence of	is a characteristic of			amino acid repeats		adhesins	GP	bacterial			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_17_5842_s_290	15317790	A characteristic of bacterial adhesins that bind to eukaryotic extracellular matrix proteins is the presence of amino acid repeats ( ).	bind
33849	1	9396	6	NULL	NULL	0	NULL	adhesins	NULL	bacterial	bind	NULL				extracellular matrix proteins	NULL	eukaryotic			NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_17_5842_s_290	15317790	A characteristic of bacterial adhesins that bind to eukaryotic extracellular matrix proteins is the presence of amino acid repeats ( ).	bind
48134	2	9396	6	10	NULL	0	NULL		NULL	presence of	is characteristic of	NULL		aminoacid repeats		adhesins	NULL	bacterial			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_17_5842_s_290	15317790	A characteristic of bacterial adhesins that bind to eukaryotic extracellular matrix proteins is the presence of amino acid repeats ( ).	bind
41034	1	9397	5	13	NULL	NULL	NULL	motor	GP		released from					F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_31701_s_133	10882730	A characteristic of myosin V is the ability to release the motor from F-actin by activating the Ca2+-dependent Mg-ATPase found in the actin binding head of myosin V ( 14,  22).	bind
41035	2	9397	5	13	NULL	NULL	NULL	statement 1	Process		is a characteristic of					myosin V	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_31701_s_133	10882730	A characteristic of myosin V is the ability to release the motor from F-actin by activating the Ca2+-dependent Mg-ATPase found in the actin binding head of myosin V ( 14,  22).	bind
41036	3	9397	5	13	NULL	NULL	NULL	myosin V	GP		activates					Mg-ATPase	GP	Ca2+-dependent			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_31701_s_133	10882730	A characteristic of myosin V is the ability to release the motor from F-actin by activating the Ca2+-dependent Mg-ATPase found in the actin binding head of myosin V ( 14,  22).	bind
41037	4	9397	5	13	NULL	NULL	NULL	Mg-ATPase	GP	Ca2+-dependent	is present in					myosin V	GP		actin binding head		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_31701_s_133	10882730	A characteristic of myosin V is the ability to release the motor from F-actin by activating the Ca2+-dependent Mg-ATPase found in the actin binding head of myosin V ( 14,  22).	bind
41038	5	9397	5	13	NULL	NULL	NULL	statement 3	Process		leads to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_31701_s_133	10882730	A characteristic of myosin V is the ability to release the motor from F-actin by activating the Ca2+-dependent Mg-ATPase found in the actin binding head of myosin V ( 14,  22).	bind
33850	1	9397	6	NULL	NULL	0	NULL	F-actin	NULL		releases	NULL				motor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_41_31701_s_133	10882730	A characteristic of myosin V is the ability to release the motor from F-actin by activating the Ca2+-dependent Mg-ATPase found in the actin binding head of myosin V ( 14,  22).	bind
33851	2	9397	6	NULL	NULL	0	NULL	myosin V	NULL		performs	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_41_31701_s_133	10882730	A characteristic of myosin V is the ability to release the motor from F-actin by activating the Ca2+-dependent Mg-ATPase found in the actin binding head of myosin V ( 14,  22).	bind
33852	3	9397	6	NULL	NULL	0	NULL	Myosin V	NULL		contains	NULL		actin binding head		Mg-ATPase	NULL	Ca2+-dependent 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_41_31701_s_133	10882730	A characteristic of myosin V is the ability to release the motor from F-actin by activating the Ca2+-dependent Mg-ATPase found in the actin binding head of myosin V ( 14,  22).	bind
33853	4	9397	6	NULL	NULL	0	NULL	statement 2	NULL		occurs by 	NULL				Mg-ATPase	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_41_31701_s_133	10882730	A characteristic of myosin V is the ability to release the motor from F-actin by activating the Ca2+-dependent Mg-ATPase found in the actin binding head of myosin V ( 14,  22).	bind
41039	1	9398	5	13	NULL	NULL	NULL	gamma-carboxylate	Chemical		 interacts with			 Glu-361		arginine	AminoAcid		guanidinium of 		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_10_6114_s_172	9045621	A charge interaction between gamma-carboxylate of Glu-361 and the guanidinium of arginine provides the major stabilization energy for the enzyme-substrate complex, as replacement of Glu-361 by a glutamine also removed L-arginine binding activity.	bind
41040	2	9398	5	13	NULL	NULL	NULL	statement 1	Process		provide					enzyme-substrate complex	GP	major stabilization energy of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_10_6114_s_172	9045621	A charge interaction between gamma-carboxylate of Glu-361 and the guanidinium of arginine provides the major stabilization energy for the enzyme-substrate complex, as replacement of Glu-361 by a glutamine also removed L-arginine binding activity.	bind
41041	3	9398	5	NULL	NULL	0	NULL		NULL		is replaced by	NULL		Glu-361			NULL		glutamine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_10_6114_s_172	9045621	A charge interaction between gamma-carboxylate of Glu-361 and the guanidinium of arginine provides the major stabilization energy for the enzyme-substrate complex, as replacement of Glu-361 by a glutamine also removed L-arginine binding activity.	bind
41042	4	9398	5	13	NULL	NULL	NULL	statement 3	Process		removed							binding activity of	L-arginine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_10_6114_s_172	9045621	A charge interaction between gamma-carboxylate of Glu-361 and the guanidinium of arginine provides the major stabilization energy for the enzyme-substrate complex, as replacement of Glu-361 by a glutamine also removed L-arginine binding activity.	bind
33944	1	9398	6	NULL	NULL	0	NULL	gamma-carboxylate	NULL		interacts with	NULL		Glu-361		arginine	NULL		guanidinium		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_10_6114_s_172	9045621	A charge interaction between gamma-carboxylate of Glu-361 and the guanidinium of arginine provides the major stabilization energy for the enzyme-substrate complex, as replacement of Glu-361 by a glutamine also removed L-arginine binding activity.	bind
58480	2	9398	6	10	NULL	0	NULL	statement 1			provide					enzyme-substrate complex		major stabilization energy for			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_10_6114_s_172	9045621	A charge interaction between gamma-carboxylate of Glu-361 and the guanidinium of arginine provides the major stabilization energy for the enzyme-substrate complex, as replacement of Glu-361 by a glutamine also removed L-arginine binding activity.	bind
58481	3	9398	6	10	NULL	0	NULL				replaced by			Glu-361					glutamine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_10_6114_s_172	9045621	A charge interaction between gamma-carboxylate of Glu-361 and the guanidinium of arginine provides the major stabilization energy for the enzyme-substrate complex, as replacement of Glu-361 by a glutamine also removed L-arginine binding activity.	bind
58482	4	9398	6	10	NULL	0	NULL	statement 3			removes					L-arginine		binding activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_10_6114_s_172	9045621	A charge interaction between gamma-carboxylate of Glu-361 and the guanidinium of arginine provides the major stabilization energy for the enzyme-substrate complex, as replacement of Glu-361 by a glutamine also removed L-arginine binding activity.	bind
41043	1	9399	5	13	NULL	NULL	NULL	Cc	GP		is					positively charged	Chemical	highly			NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_22_11928_s_108	11035811	A charged species may disrupt the binding of Cc and Apaf-1 through ionic interactions, because Cc and Apaf-1 are highly positively and negatively charged, respectively.	bind
41044	2	9399	5	13	NULL	NULL	NULL	Apaf-1	GP		is					negatively charged	Chemical	highly			NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_22_11928_s_108	11035811	A charged species may disrupt the binding of Cc and Apaf-1 through ionic interactions, because Cc and Apaf-1 are highly positively and negatively charged, respectively.	bind
41045	3	9399	5	13	NULL	NULL	NULL	Cc	GP		bind					Apaf-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_22_11928_s_108	11035811	A charged species may disrupt the binding of Cc and Apaf-1 through ionic interactions, because Cc and Apaf-1 are highly positively and negatively charged, respectively.	bind
41046	4	9399	5	13	NULL	NULL	NULL	charged species	Chemical		disrupt		may			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_22_11928_s_108	11035811	A charged species may disrupt the binding of Cc and Apaf-1 through ionic interactions, because Cc and Apaf-1 are highly positively and negatively charged, respectively.	bind
41047	5	9399	5	13	NULL	NULL	NULL	statement 4	Process		occurs through					ionic interactions	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_22_11928_s_108	11035811	A charged species may disrupt the binding of Cc and Apaf-1 through ionic interactions, because Cc and Apaf-1 are highly positively and negatively charged, respectively.	bind
33854	1	9399	6	NULL	NULL	0	NULL	Cc	NULL	highly positively charged	bind	NULL				Apaf-1	NULL	highly negatively charged			NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_22_11928_s_108	11035811	A charged species may disrupt the binding of Cc and Apaf-1 through ionic interactions, because Cc and Apaf-1 are highly positively and negatively charged, respectively.	bind
33855	2	9399	6	NULL	NULL	0	NULL	charged species	NULL		disrupts	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_22_11928_s_108	11035811	A charged species may disrupt the binding of Cc and Apaf-1 through ionic interactions, because Cc and Apaf-1 are highly positively and negatively charged, respectively.	bind
33856	3	9399	6	NULL	NULL	0	NULL	statement 2	NULL		occurs through	NULL				ionic interactions	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_22_11928_s_108	11035811	A charged species may disrupt the binding of Cc and Apaf-1 through ionic interactions, because Cc and Apaf-1 are highly positively and negatively charged, respectively.	bind
41048	1	9402	5	13	NULL	NULL	NULL	CD80	GP		is a type of					co-stimulating molecule	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_6_333_s_112	10744980	A chicken homologue of the co-stimulating molecule CD80 which binds to mammalian CTLA-4.	bind
41049	2	9402	5	13	NULL	NULL	NULL	CD80	GP	chicken homologue	bind					CTLA-4	GP	mammalian			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_6_333_s_112	10744980	A chicken homologue of the co-stimulating molecule CD80 which binds to mammalian CTLA-4.	bind
39493	1	9402	7	10	NULL	0	NULL	CD80	NULL	chicken homologue	bind	NULL				CTLA-4	NULL	mammalian			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_6_333_s_112	10744980	A chicken homologue of the co-stimulating molecule CD80 which binds to mammalian CTLA-4.	bind
39494	2	9402	7	NULL	NULL	0	NULL	CD80	NULL		is a type of	NULL				co-stimulating molecule	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_6_333_s_112	10744980	A chicken homologue of the co-stimulating molecule CD80 which binds to mammalian CTLA-4.	bind
42995	1	9403	5	13	NULL	NULL	NULL	chimera	GP		consists of					nNOS	GP		heme domain		NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_28_12730215_s_6	12730215	A chimera consisting  of the nNOS heme domain and FMN binding subdomain and the CYPOR FAD binding  subdomain catalyzed significantly increased rates of cytochrome c reduction  in the absence of CaM and of NO synthesis in its presence.	bind
42996	2	9403	5	13	NULL	NULL	NULL	chimera	GP		consists of								FMN binding subdomain		NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_28_12730215_s_6	12730215	A chimera consisting  of the nNOS heme domain and FMN binding subdomain and the CYPOR FAD binding  subdomain catalyzed significantly increased rates of cytochrome c reduction  in the absence of CaM and of NO synthesis in its presence.	bind
42997	3	9403	5	13	NULL	NULL	NULL	chimera	GP		consists of					CYPOR	GP		FAD binding subdomain		NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_28_12730215_s_6	12730215	A chimera consisting  of the nNOS heme domain and FMN binding subdomain and the CYPOR FAD binding  subdomain catalyzed significantly increased rates of cytochrome c reduction  in the absence of CaM and of NO synthesis in its presence.	bind
43009	4	9403	5	13	NULL	NULL	NULL	cytochrome c	GP		undergoes					reduction	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_28_12730215_s_6	12730215	A chimera consisting  of the nNOS heme domain and FMN binding subdomain and the CYPOR FAD binding  subdomain catalyzed significantly increased rates of cytochrome c reduction  in the absence of CaM and of NO synthesis in its presence.	bind
43010	5	9403	5	13	NULL	NULL	NULL	statement 4	Process		in the absence of					CaM	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_28_12730215_s_6	12730215	A chimera consisting  of the nNOS heme domain and FMN binding subdomain and the CYPOR FAD binding  subdomain catalyzed significantly increased rates of cytochrome c reduction  in the absence of CaM and of NO synthesis in its presence.	bind
43011	6	9403	5	13	NULL	NULL	NULL	statement 1	Process		catalyze		significantly			statement 4	Process	increased rates of			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_28_12730215_s_6	12730215	A chimera consisting  of the nNOS heme domain and FMN binding subdomain and the CYPOR FAD binding  subdomain catalyzed significantly increased rates of cytochrome c reduction  in the absence of CaM and of NO synthesis in its presence.	bind
43012	7	9403	5	13	NULL	NULL	NULL	statement 2	Process		catalyze		significantly			statement 4	Process	increased rates of			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_28_12730215_s_6	12730215	A chimera consisting  of the nNOS heme domain and FMN binding subdomain and the CYPOR FAD binding  subdomain catalyzed significantly increased rates of cytochrome c reduction  in the absence of CaM and of NO synthesis in its presence.	bind
43013	8	9403	5	13	NULL	NULL	NULL	statement 3	Process		catalyze		significantly			statement 4	Process	increased rates of			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_28_12730215_s_6	12730215	A chimera consisting  of the nNOS heme domain and FMN binding subdomain and the CYPOR FAD binding  subdomain catalyzed significantly increased rates of cytochrome c reduction  in the absence of CaM and of NO synthesis in its presence.	bind
43014	9	9403	5	13	NULL	NULL	NULL	statement 1	Process		catalyze					NO	Chemical	synthesis of			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_28_12730215_s_6	12730215	A chimera consisting  of the nNOS heme domain and FMN binding subdomain and the CYPOR FAD binding  subdomain catalyzed significantly increased rates of cytochrome c reduction  in the absence of CaM and of NO synthesis in its presence.	bind
43015	10	9403	5	13	NULL	NULL	NULL	statement 9	Process		in the presence of					CaM	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_28_12730215_s_6	12730215	A chimera consisting  of the nNOS heme domain and FMN binding subdomain and the CYPOR FAD binding  subdomain catalyzed significantly increased rates of cytochrome c reduction  in the absence of CaM and of NO synthesis in its presence.	bind
43016	11	9403	5	13	NULL	NULL	NULL	statement 2	Process		catalyze					NO	Chemical	synthesis of			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_28_12730215_s_6	12730215	A chimera consisting  of the nNOS heme domain and FMN binding subdomain and the CYPOR FAD binding  subdomain catalyzed significantly increased rates of cytochrome c reduction  in the absence of CaM and of NO synthesis in its presence.	bind
43017	12	9403	5	13	NULL	NULL	NULL	statement 11	Process		in the presence of					CaM	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_28_12730215_s_6	12730215	A chimera consisting  of the nNOS heme domain and FMN binding subdomain and the CYPOR FAD binding  subdomain catalyzed significantly increased rates of cytochrome c reduction  in the absence of CaM and of NO synthesis in its presence.	bind
43018	13	9403	5	13	NULL	NULL	NULL	statement 3	Process		catalyze					NO	Chemical	synthesis of			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_28_12730215_s_6	12730215	A chimera consisting  of the nNOS heme domain and FMN binding subdomain and the CYPOR FAD binding  subdomain catalyzed significantly increased rates of cytochrome c reduction  in the absence of CaM and of NO synthesis in its presence.	bind
43019	14	9403	5	13	NULL	NULL	NULL	statement 13	Process		in the presence of					CaM	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_28_12730215_s_6	12730215	A chimera consisting  of the nNOS heme domain and FMN binding subdomain and the CYPOR FAD binding  subdomain catalyzed significantly increased rates of cytochrome c reduction  in the absence of CaM and of NO synthesis in its presence.	bind
39495	1	9403	7	NULL	NULL	0	NULL	 chimera	NULL		consist of	NULL					NULL		nNOS heme domain		NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_28_12730215_s_6	12730215	A chimera consisting  of the nNOS heme domain and FMN binding subdomain and the CYPOR FAD binding  subdomain catalyzed significantly increased rates of cytochrome c reduction  in the absence of CaM and of NO synthesis in its presence.	bind
39496	2	9403	7	NULL	NULL	0	NULL	chimera	NULL		consist of	NULL					NULL		FMN binding subdomain		NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_28_12730215_s_6	12730215	A chimera consisting  of the nNOS heme domain and FMN binding subdomain and the CYPOR FAD binding  subdomain catalyzed significantly increased rates of cytochrome c reduction  in the absence of CaM and of NO synthesis in its presence.	bind
39497	3	9403	7	10	NULL	0	NULL	chimera			consist of					CYPOR			FAD binding subdomain		NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_28_12730215_s_6	12730215	A chimera consisting  of the nNOS heme domain and FMN binding subdomain and the CYPOR FAD binding  subdomain catalyzed significantly increased rates of cytochrome c reduction  in the absence of CaM and of NO synthesis in its presence.	bind
39498	4	9403	7	NULL	NULL	0	NULL	statement 1	NULL		occur simultaneously with	NULL				statement 2 	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_28_12730215_s_6	12730215	A chimera consisting  of the nNOS heme domain and FMN binding subdomain and the CYPOR FAD binding  subdomain catalyzed significantly increased rates of cytochrome c reduction  in the absence of CaM and of NO synthesis in its presence.	bind
39499	6	9403	7	NULL	NULL	0	NULL	chimera	NULL		increase	NULL				cytochrome c	NULL	reduction of			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_28_12730215_s_6	12730215	A chimera consisting  of the nNOS heme domain and FMN binding subdomain and the CYPOR FAD binding  subdomain catalyzed significantly increased rates of cytochrome c reduction  in the absence of CaM and of NO synthesis in its presence.	bind
39500	7	9403	7	NULL	NULL	0	NULL	statement 6	NULL		in absence of	NULL				CaM	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_28_12730215_s_6	12730215	A chimera consisting  of the nNOS heme domain and FMN binding subdomain and the CYPOR FAD binding  subdomain catalyzed significantly increased rates of cytochrome c reduction  in the absence of CaM and of NO synthesis in its presence.	bind
39501	8	9403	7	NULL	NULL	0	NULL	chimera	NULL		increase	NULL				NO	NULL	synthesis of			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_28_12730215_s_6	12730215	A chimera consisting  of the nNOS heme domain and FMN binding subdomain and the CYPOR FAD binding  subdomain catalyzed significantly increased rates of cytochrome c reduction  in the absence of CaM and of NO synthesis in its presence.	bind
39502	9	9403	7	NULL	NULL	0	NULL	statement 8	NULL		in presence of	NULL				CaM	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_28_12730215_s_6	12730215	A chimera consisting  of the nNOS heme domain and FMN binding subdomain and the CYPOR FAD binding  subdomain catalyzed significantly increased rates of cytochrome c reduction  in the absence of CaM and of NO synthesis in its presence.	bind
40403	5	9403	7	NULL	NULL	0	NULL	statement 1	NULL		occur simultaneously with	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_28_12730215_s_6	12730215	A chimera consisting  of the nNOS heme domain and FMN binding subdomain and the CYPOR FAD binding  subdomain catalyzed significantly increased rates of cytochrome c reduction  in the absence of CaM and of NO synthesis in its presence.	bind
43025	1	9404	5	13	NULL	NULL	NULL	chimera	GP		consists of					MKP-3	GP		N-terminal half		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_9323_s_6	9535927	A chimera consisting of the N-terminal half of MKP-3 with the C-terminal catalytic core of M3-6 also bound tightly to ERK1 but not to JNK3/SAPKbeta.	bind
43026	2	9404	5	13	NULL	NULL	NULL	chimera	GP		consists of					M3-6	GP		C-terminal catalytic core		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_9323_s_6	9535927	A chimera consisting of the N-terminal half of MKP-3 with the C-terminal catalytic core of M3-6 also bound tightly to ERK1 but not to JNK3/SAPKbeta.	bind
43041	3	9404	5	13	NULL	NULL	NULL	statement 1	GP		bind		tightly			ERK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_9323_s_6	9535927	A chimera consisting of the N-terminal half of MKP-3 with the C-terminal catalytic core of M3-6 also bound tightly to ERK1 but not to JNK3/SAPKbeta.	bind
43042	4	9404	5	13	NULL	NULL	NULL	statement 2	GP		bind		tightly			ERK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_9323_s_6	9535927	A chimera consisting of the N-terminal half of MKP-3 with the C-terminal catalytic core of M3-6 also bound tightly to ERK1 but not to JNK3/SAPKbeta.	bind
43043	5	9404	5	13	NULL	NULL	NULL	statement 1	GP		does not bind					JNK3/SAPKbeta	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_9323_s_6	9535927	A chimera consisting of the N-terminal half of MKP-3 with the C-terminal catalytic core of M3-6 also bound tightly to ERK1 but not to JNK3/SAPKbeta.	bind
43044	6	9404	5	13	NULL	NULL	NULL	statement 2	GP		does not bind					JNK3/SAPKbeta	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_9323_s_6	9535927	A chimera consisting of the N-terminal half of MKP-3 with the C-terminal catalytic core of M3-6 also bound tightly to ERK1 but not to JNK3/SAPKbeta.	bind
39503	1	9404	7	NULL	NULL	0	NULL	 chimera	NULL		consist of	NULL				MKP-3	NULL		N-terminal half of		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_15_9323_s_6	9535927	A chimera consisting of the N-terminal half of MKP-3 with the C-terminal catalytic core of M3-6 also bound tightly to ERK1 but not to JNK3/SAPKbeta.	bind
39504	2	9404	7	NULL	NULL	0	NULL	chimera	NULL		consist of	NULL				M3-6	NULL		C-terminal catalytic core 		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_15_9323_s_6	9535927	A chimera consisting of the N-terminal half of MKP-3 with the C-terminal catalytic core of M3-6 also bound tightly to ERK1 but not to JNK3/SAPKbeta.	bind
39505	3	9404	7	NULL	NULL	0	NULL	statement 1	NULL		is composed of	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_15_9323_s_6	9535927	A chimera consisting of the N-terminal half of MKP-3 with the C-terminal catalytic core of M3-6 also bound tightly to ERK1 but not to JNK3/SAPKbeta.	bind
39506	4	9404	7	NULL	NULL	0	NULL	statement 3	NULL		binds	NULL	tightly			ERK1 	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_15_9323_s_6	9535927	A chimera consisting of the N-terminal half of MKP-3 with the C-terminal catalytic core of M3-6 also bound tightly to ERK1 but not to JNK3/SAPKbeta.	bind
39507	5	9404	7	NULL	NULL	0	NULL	statement 3	NULL		does not bind	NULL				JNK3/SAPKbeta	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_15_9323_s_6	9535927	A chimera consisting of the N-terminal half of MKP-3 with the C-terminal catalytic core of M3-6 also bound tightly to ERK1 but not to JNK3/SAPKbeta.	bind
43020	1	9406	5	13	NULL	NULL	NULL	ChiAVD	GP		is a type of					chimeric avidin protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_10228_s_9	15649900	A chimeric avidin protein, ChiAVD, containing a 21-amino acid segment of AVR4 was found to be significantly more stable ( Tm = 96.5  degrees C) than native avidin ( Tm = 83.5  degrees C), and its biotin-binding properties resembled those of AVR4.	bind
43021	2	9406	5	13	NULL	NULL	NULL	ChiAVD	GP		contains					AVR4	GP	21-amino acid segment of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_10228_s_9	15649900	A chimeric avidin protein, ChiAVD, containing a 21-amino acid segment of AVR4 was found to be significantly more stable ( Tm = 96.5  degrees C) than native avidin ( Tm = 83.5  degrees C), and its biotin-binding properties resembled those of AVR4.	bind
43022	3	9406	5	13	NULL	NULL	NULL	statement 2	GP		more stable than		significantly			avidin	GP	native			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_10228_s_9	15649900	A chimeric avidin protein, ChiAVD, containing a 21-amino acid segment of AVR4 was found to be significantly more stable ( Tm = 96.5  degrees C) than native avidin ( Tm = 83.5  degrees C), and its biotin-binding properties resembled those of AVR4.	bind
43023	4	9406	5	13	NULL	NULL	NULL	ChiAVD	GP		bind					biotin	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_10228_s_9	15649900	A chimeric avidin protein, ChiAVD, containing a 21-amino acid segment of AVR4 was found to be significantly more stable ( Tm = 96.5  degrees C) than native avidin ( Tm = 83.5  degrees C), and its biotin-binding properties resembled those of AVR4.	bind
46826	5	9406	5	13	NULL	NULL	NULL	AVR4	GP		bind					biotin	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_10228_s_9	15649900	A chimeric avidin protein, ChiAVD, containing a 21-amino acid segment of AVR4 was found to be significantly more stable ( Tm = 96.5  degrees C) than native avidin ( Tm = 83.5  degrees C), and its biotin-binding properties resembled those of AVR4.	bind
46827	6	9406	5	13	NULL	NULL	NULL	statement 4	Process		is similar to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_10228_s_9	15649900	A chimeric avidin protein, ChiAVD, containing a 21-amino acid segment of AVR4 was found to be significantly more stable ( Tm = 96.5  degrees C) than native avidin ( Tm = 83.5  degrees C), and its biotin-binding properties resembled those of AVR4.	bind
39508	1	9406	7	NULL	NULL	0	NULL	ChiAVD	NULL		is	NULL				chimeric avidin protein	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_11_10228_s_9	15649900	A chimeric avidin protein, ChiAVD, containing a 21-amino acid segment of AVR4 was found to be significantly more stable ( Tm = 96.5  degrees C) than native avidin ( Tm = 83.5  degrees C), and its biotin-binding properties resembled those of AVR4.	bind
39509	2	9406	7	NULL	NULL	0	NULL	ChiAVD	NULL		contains	NULL				AVR4	NULL		 21-amino acid segment		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_11_10228_s_9	15649900	A chimeric avidin protein, ChiAVD, containing a 21-amino acid segment of AVR4 was found to be significantly more stable ( Tm = 96.5  degrees C) than native avidin ( Tm = 83.5  degrees C), and its biotin-binding properties resembled those of AVR4.	bind
39510	3	9406	7	10	NULL	0	NULL	ChiAVD			is more stable than		significantly			avidin		native			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_10228_s_9	15649900	A chimeric avidin protein, ChiAVD, containing a 21-amino acid segment of AVR4 was found to be significantly more stable ( Tm = 96.5  degrees C) than native avidin ( Tm = 83.5  degrees C), and its biotin-binding properties resembled those of AVR4.	bind
39511	4	9406	7	NULL	NULL	0	NULL	ChiAVD	NULL		bind	NULL				biotin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_11_10228_s_9	15649900	A chimeric avidin protein, ChiAVD, containing a 21-amino acid segment of AVR4 was found to be significantly more stable ( Tm = 96.5  degrees C) than native avidin ( Tm = 83.5  degrees C), and its biotin-binding properties resembled those of AVR4.	bind
39512	5	9406	7	10	NULL	0	NULL	AVR4	NULL		bind	NULL				biotin	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_10228_s_9	15649900	A chimeric avidin protein, ChiAVD, containing a 21-amino acid segment of AVR4 was found to be significantly more stable ( Tm = 96.5  degrees C) than native avidin ( Tm = 83.5  degrees C), and its biotin-binding properties resembled those of AVR4.	bind
46828	6	9406	7	10	NULL	0	NULL	statement 4	NULL		resembles	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_11_10228_s_9	15649900	A chimeric avidin protein, ChiAVD, containing a 21-amino acid segment of AVR4 was found to be significantly more stable ( Tm = 96.5  degrees C) than native avidin ( Tm = 83.5  degrees C), and its biotin-binding properties resembled those of AVR4.	bind
43054	2	9407	5	13	NULL	NULL	NULL	chimeric beta4 integrin	GP		is replaced with			SDL sequence		beta1 integrin	GP	corresponding	SDL sequence		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49406_s_12	14512419	A chimeric beta4 integrin in which the indicated SDL sequence had been replaced with the corresponding sequence from the beta1 integrin failed to bind hCLCA2.	bind
43055	3	9407	5	13	NULL	NULL	NULL	statement 2	GP		does not bind					hCLCA2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49406_s_12	14512419	A chimeric beta4 integrin in which the indicated SDL sequence had been replaced with the corresponding sequence from the beta1 integrin failed to bind hCLCA2.	bind
39513	1	9407	7	10	NULL	0	NULL	chimeric beta4 integrin			is replaced with			SDL sequence		beta1 integrin		corresponding	SDL sequence		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49406_s_12	14512419	A chimeric beta4 integrin in which the indicated SDL sequence had been replaced with the corresponding sequence from the beta1 integrin failed to bind hCLCA2.	bind
39514	2	9407	7	NULL	NULL	0	NULL	chimeric beta4 integrin	NULL		fails to bind	NULL				hCLCA2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49406_s_12	14512419	A chimeric beta4 integrin in which the indicated SDL sequence had been replaced with the corresponding sequence from the beta1 integrin failed to bind hCLCA2.	bind
43056	1	9408	5	13	NULL	NULL	NULL	VEGF	GP	chimeric ligand of	fused to					alkaline phosphatase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_16_19_6089_s_172	8815891	A chimeric ligand of VEGF fused to alkaline phosphatase binds to [[ retinal progenitor cells           ]]Flk-1 receptor has been reported to bind VEGF with high affinity.	bind
43057	2	9408	5	13	NULL	NULL	NULL	statement 1	GP		bind					progenitor cells	Cell	retinal			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_16_19_6089_s_172	8815891	A chimeric ligand of VEGF fused to alkaline phosphatase binds to [[ retinal progenitor cells           ]]Flk-1 receptor has been reported to bind VEGF with high affinity.	bind
43058	3	9408	5	13	NULL	NULL	NULL	Flk-1 receptor	GP		bind		high affinity			VEGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_16_19_6089_s_172	8815891	A chimeric ligand of VEGF fused to alkaline phosphatase binds to [[ retinal progenitor cells           ]]Flk-1 receptor has been reported to bind VEGF with high affinity.	bind
39619	1	9408	7	10	NULL	0	NULL	VEGF 	NULL	chimeric ligand of 	fused to	NULL				alkaline phosphatase	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_16_19_6089_s_172	8815891	A chimeric ligand of VEGF fused to alkaline phosphatase binds to [[ retinal progenitor cells           ]]Flk-1 receptor has been reported to bind VEGF with high affinity.	bind
39620	2	9408	7	10	NULL	0	NULL	statement 1			binds to					progenitor cells		retinal 			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_16_19_6089_s_172	8815891	A chimeric ligand of VEGF fused to alkaline phosphatase binds to [[ retinal progenitor cells           ]]Flk-1 receptor has been reported to bind VEGF with high affinity.	bind
39621	3	9408	7	NULL	NULL	0	NULL	Flk-1 receptor	NULL		bind	NULL	high affinity			VEGF	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_16_19_6089_s_172	8815891	A chimeric ligand of VEGF fused to alkaline phosphatase binds to [[ retinal progenitor cells           ]]Flk-1 receptor has been reported to bind VEGF with high affinity.	bind
43059	1	9409	5	13	NULL	NULL	NULL	TTR	GP	crocodile	is replaced by			N-terminal end		TTR	GP	frog			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_25_26411_s_91	15082720	A chimeric molecule generated from crocodile TTR, in which the N-terminal end was replaced by that from frog, was shown to differ in both the specificity and affinity of T4 and T3 binding.	bind
43060	2	9409	5	13	NULL	NULL	NULL	chimeric molecule	GP		is generated from					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_25_26411_s_91	15082720	A chimeric molecule generated from crocodile TTR, in which the N-terminal end was replaced by that from frog, was shown to differ in both the specificity and affinity of T4 and T3 binding.	bind
43071	3	9409	5	13	NULL	NULL	NULL	statement 2	GP		bind					T4	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_25_26411_s_91	15082720	A chimeric molecule generated from crocodile TTR, in which the N-terminal end was replaced by that from frog, was shown to differ in both the specificity and affinity of T4 and T3 binding.	bind
43072	4	9409	5	13	NULL	NULL	NULL	statement 2	GP		bind					T3	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_25_26411_s_91	15082720	A chimeric molecule generated from crocodile TTR, in which the N-terminal end was replaced by that from frog, was shown to differ in both the specificity and affinity of T4 and T3 binding.	bind
43073	5	9409	5	13	NULL	NULL	NULL	statement 3	Process		differ in					statement 4	Process	specificity of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_25_26411_s_91	15082720	A chimeric molecule generated from crocodile TTR, in which the N-terminal end was replaced by that from frog, was shown to differ in both the specificity and affinity of T4 and T3 binding.	bind
43074	6	9409	5	13	NULL	NULL	NULL	statement 3	Process		differ in					statement 4	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_25_26411_s_91	15082720	A chimeric molecule generated from crocodile TTR, in which the N-terminal end was replaced by that from frog, was shown to differ in both the specificity and affinity of T4 and T3 binding.	bind
39622	1	9409	7	10	NULL	0	NULL	TTR		crocodile	is replaced by			N-terminal end		TTR		frog			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_25_26411_s_91	15082720	A chimeric molecule generated from crocodile TTR, in which the N-terminal end was replaced by that from frog, was shown to differ in both the specificity and affinity of T4 and T3 binding.	bind
39623	2	9409	7	10	NULL	0	NULL	chimeric molecule			is generated from					statement 1					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_25_26411_s_91	15082720	A chimeric molecule generated from crocodile TTR, in which the N-terminal end was replaced by that from frog, was shown to differ in both the specificity and affinity of T4 and T3 binding.	bind
39624	3	9409	7	10	NULL	0	NULL	statement 2			bind					T4					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_25_26411_s_91	15082720	A chimeric molecule generated from crocodile TTR, in which the N-terminal end was replaced by that from frog, was shown to differ in both the specificity and affinity of T4 and T3 binding.	bind
39625	4	9409	7	10	NULL	0	NULL	statement 2			bind					T3					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_25_26411_s_91	15082720	A chimeric molecule generated from crocodile TTR, in which the N-terminal end was replaced by that from frog, was shown to differ in both the specificity and affinity of T4 and T3 binding.	bind
40405	5	9409	7	10	NULL	0	NULL	statement 3			differ in					statement 4		specificity of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_25_26411_s_91	15082720	A chimeric molecule generated from crocodile TTR, in which the N-terminal end was replaced by that from frog, was shown to differ in both the specificity and affinity of T4 and T3 binding.	bind
46829	6	9409	7	10	NULL	0	NULL	statement 3			differ in					statement 4		affinity of 			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_25_26411_s_91	15082720	A chimeric molecule generated from crocodile TTR, in which the N-terminal end was replaced by that from frog, was shown to differ in both the specificity and affinity of T4 and T3 binding.	bind
43045	1	9410	5	13	NULL	NULL	NULL	Sec9p	GP		bind			helix		Sso1/2p	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_genetics_166_1_15020409_s_5	15020409	A chimeric molecule, in which the helices of Sec9p  that bind to Sso1/2p and Snc1/2p are replaced with the homologous regions  of Spo20p, will not support vesicle fusion in vegetative cells.	bind
43046	2	9410	5	13	NULL	NULL	NULL	Sec9p	GP		bind			helix		Snc1/2p	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_genetics_166_1_15020409_s_5	15020409	A chimeric molecule, in which the helices of Sec9p  that bind to Sso1/2p and Snc1/2p are replaced with the homologous regions  of Spo20p, will not support vesicle fusion in vegetative cells.	bind
43047	3	9410	5	13	NULL	NULL	NULL	statement 1	GP		is replaced with					Spo20p	GP	homologous regions of			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_genetics_166_1_15020409_s_5	15020409	A chimeric molecule, in which the helices of Sec9p  that bind to Sso1/2p and Snc1/2p are replaced with the homologous regions  of Spo20p, will not support vesicle fusion in vegetative cells.	bind
43048	4	9410	5	13	NULL	NULL	NULL	statement 2	GP		is replaced with					Spo20p	GP	homologous regions of			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_genetics_166_1_15020409_s_5	15020409	A chimeric molecule, in which the helices of Sec9p  that bind to Sso1/2p and Snc1/2p are replaced with the homologous regions  of Spo20p, will not support vesicle fusion in vegetative cells.	bind
43049	5	9410	5	13	NULL	NULL	NULL	chimera	GP		consists of					statement 3	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_genetics_166_1_15020409_s_5	15020409	A chimeric molecule, in which the helices of Sec9p  that bind to Sso1/2p and Snc1/2p are replaced with the homologous regions  of Spo20p, will not support vesicle fusion in vegetative cells.	bind
43050	6	9410	5	13	NULL	NULL	NULL	chimera	GP		consists of					statement 4	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_genetics_166_1_15020409_s_5	15020409	A chimeric molecule, in which the helices of Sec9p  that bind to Sso1/2p and Snc1/2p are replaced with the homologous regions  of Spo20p, will not support vesicle fusion in vegetative cells.	bind
43051	7	9410	5	13	NULL	NULL	NULL	statement 5	Process		does not support					vesicle	CellComponent	fusion of			NULL	in vegetative cells	NULL	NULL	NULL	NULL	abs-batch0650-0679_genetics_166_1_15020409_s_5	15020409	A chimeric molecule, in which the helices of Sec9p  that bind to Sso1/2p and Snc1/2p are replaced with the homologous regions  of Spo20p, will not support vesicle fusion in vegetative cells.	bind
43052	8	9410	5	13	NULL	NULL	NULL	statement 6	Process		does not support					vesicle	CellComponent	fusion of			NULL	in vegetative cells	NULL	NULL	NULL	NULL	abs-batch0650-0679_genetics_166_1_15020409_s_5	15020409	A chimeric molecule, in which the helices of Sec9p  that bind to Sso1/2p and Snc1/2p are replaced with the homologous regions  of Spo20p, will not support vesicle fusion in vegetative cells.	bind
39626	1	9410	7	NULL	NULL	0	NULL	Sec9p	NULL		bind	NULL		helix		Sso1/2p	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_genetics_166_1_15020409_s_5	15020409	A chimeric molecule, in which the helices of Sec9p  that bind to Sso1/2p and Snc1/2p are replaced with the homologous regions  of Spo20p, will not support vesicle fusion in vegetative cells.	bind
39627	2	9410	7	NULL	NULL	0	NULL	Sec9p	NULL		bind	NULL		helix		Snc1/2p	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_genetics_166_1_15020409_s_5	15020409	A chimeric molecule, in which the helices of Sec9p  that bind to Sso1/2p and Snc1/2p are replaced with the homologous regions  of Spo20p, will not support vesicle fusion in vegetative cells.	bind
39628	3	9410	7	NULL	NULL	0	NULL	statement 1	NULL		is replaced with	NULL				Spo20p	NULL	homologous regions of			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_genetics_166_1_15020409_s_5	15020409	A chimeric molecule, in which the helices of Sec9p  that bind to Sso1/2p and Snc1/2p are replaced with the homologous regions  of Spo20p, will not support vesicle fusion in vegetative cells.	bind
39629	5	9410	7	NULL	NULL	0	NULL	chimeric molecule	NULL		consist of	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_genetics_166_1_15020409_s_5	15020409	A chimeric molecule, in which the helices of Sec9p  that bind to Sso1/2p and Snc1/2p are replaced with the homologous regions  of Spo20p, will not support vesicle fusion in vegetative cells.	bind
48773	4	9410	7	NULL	NULL	0	NULL	statement 2	NULL		is replaced with	NULL				Spo20p	NULL	homologous regions of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_genetics_166_1_15020409_s_5	15020409	A chimeric molecule, in which the helices of Sec9p  that bind to Sso1/2p and Snc1/2p are replaced with the homologous regions  of Spo20p, will not support vesicle fusion in vegetative cells.	bind
48774	6	9410	7	NULL	NULL	0	NULL	chimeric molecule	NULL		consist of	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_genetics_166_1_15020409_s_5	15020409	A chimeric molecule, in which the helices of Sec9p  that bind to Sso1/2p and Snc1/2p are replaced with the homologous regions  of Spo20p, will not support vesicle fusion in vegetative cells.	bind
48775	7	9410	7	NULL	NULL	0	NULL	statement 5	NULL		does not support	NULL				vesicle	NULL	fusion of			NULL	vegetative cells	0	NULL	NULL	NULL	abs-batch0650-0679_genetics_166_1_15020409_s_5	15020409	A chimeric molecule, in which the helices of Sec9p  that bind to Sso1/2p and Snc1/2p are replaced with the homologous regions  of Spo20p, will not support vesicle fusion in vegetative cells.	bind
48776	8	9410	7	NULL	NULL	0	NULL	statement 6	NULL		does not support	NULL				vesicle	NULL	fusion of			NULL	vegetative cells	0	NULL	NULL	NULL	abs-batch0650-0679_genetics_166_1_15020409_s_5	15020409	A chimeric molecule, in which the helices of Sec9p  that bind to Sso1/2p and Snc1/2p are replaced with the homologous regions  of Spo20p, will not support vesicle fusion in vegetative cells.	bind
43212	1	9412	5	13	NULL	NULL	NULL	chimeric receptor	GP		contains					GABAB	GP		ATD of R1a subunit		NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_76_1_180_s_248	10719229	A chimeric receptor containing the ATD of the GABAB R1a subunit encompassing all of the ATD except the last 40 amino acids immediately upstream of the first TMD (termed aN550) bound a GABAB receptor photoaffinity ligand, while a construct fused 60 amino acids upstream of the first TMD (termed aN530) did not bind the photoaffinity label [ 23].	bind
43213	2	9412	5	13	NULL	NULL	NULL	GABAB	GP		encompass			ATD of R1a subunit					ATD		NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_76_1_180_s_248	10719229	A chimeric receptor containing the ATD of the GABAB R1a subunit encompassing all of the ATD except the last 40 amino acids immediately upstream of the first TMD (termed aN550) bound a GABAB receptor photoaffinity ligand, while a construct fused 60 amino acids upstream of the first TMD (termed aN530) did not bind the photoaffinity label [ 23].	bind
43214	3	9412	5	13	NULL	NULL	NULL	40 amino acids	GP		upstream of		immediately						first TMD		NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_76_1_180_s_248	10719229	A chimeric receptor containing the ATD of the GABAB R1a subunit encompassing all of the ATD except the last 40 amino acids immediately upstream of the first TMD (termed aN550) bound a GABAB receptor photoaffinity ligand, while a construct fused 60 amino acids upstream of the first TMD (termed aN530) did not bind the photoaffinity label [ 23].	bind
43215	4	9412	5	13	NULL	NULL	NULL	statement 3	Process		is an exception for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_76_1_180_s_248	10719229	A chimeric receptor containing the ATD of the GABAB R1a subunit encompassing all of the ATD except the last 40 amino acids immediately upstream of the first TMD (termed aN550) bound a GABAB receptor photoaffinity ligand, while a construct fused 60 amino acids upstream of the first TMD (termed aN530) did not bind the photoaffinity label [ 23].	bind
43216	5	9412	5	13	NULL	NULL	NULL	statement 1	GP		bind					GABAB receptor photoaffinity ligand	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_76_1_180_s_248	10719229	A chimeric receptor containing the ATD of the GABAB R1a subunit encompassing all of the ATD except the last 40 amino acids immediately upstream of the first TMD (termed aN550) bound a GABAB receptor photoaffinity ligand, while a construct fused 60 amino acids upstream of the first TMD (termed aN530) did not bind the photoaffinity label [ 23].	bind
43217	6	9412	5	13	NULL	NULL	NULL	60 amino acids	GP		fused to							upstream of	first TMD		NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_76_1_180_s_248	10719229	A chimeric receptor containing the ATD of the GABAB R1a subunit encompassing all of the ATD except the last 40 amino acids immediately upstream of the first TMD (termed aN550) bound a GABAB receptor photoaffinity ligand, while a construct fused 60 amino acids upstream of the first TMD (termed aN530) did not bind the photoaffinity label [ 23].	bind
43218	7	9412	5	13	NULL	NULL	NULL	construct	GP		contains					statement 6	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_76_1_180_s_248	10719229	A chimeric receptor containing the ATD of the GABAB R1a subunit encompassing all of the ATD except the last 40 amino acids immediately upstream of the first TMD (termed aN550) bound a GABAB receptor photoaffinity ligand, while a construct fused 60 amino acids upstream of the first TMD (termed aN530) did not bind the photoaffinity label [ 23].	bind
43219	8	9412	5	13	NULL	NULL	NULL	statement 7	GP		does not bind					photoaffinity label	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_76_1_180_s_248	10719229	A chimeric receptor containing the ATD of the GABAB R1a subunit encompassing all of the ATD except the last 40 amino acids immediately upstream of the first TMD (termed aN550) bound a GABAB receptor photoaffinity ligand, while a construct fused 60 amino acids upstream of the first TMD (termed aN530) did not bind the photoaffinity label [ 23].	bind
39632	1	9412	7	10	NULL	0	NULL	chimeric receptor	NULL		contains	NULL				GABAB	NULL		ATD R1a subunit 		NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_76_1_180_s_248	10719229	A chimeric receptor containing the ATD of the GABAB R1a subunit encompassing all of the ATD except the last 40 amino acids immediately upstream of the first TMD (termed aN550) bound a GABAB receptor photoaffinity ligand, while a construct fused 60 amino acids upstream of the first TMD (termed aN530) did not bind the photoaffinity label [ 23].	bind
39707	2	9412	7	NULL	NULL	0	NULL	chimeric receptor	NULL		does not have	NULL				ATD	NULL		 last 40 amino acid upstream of first TMD		NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_76_1_180_s_248	10719229	A chimeric receptor containing the ATD of the GABAB R1a subunit encompassing all of the ATD except the last 40 amino acids immediately upstream of the first TMD (termed aN550) bound a GABAB receptor photoaffinity ligand, while a construct fused 60 amino acids upstream of the first TMD (termed aN530) did not bind the photoaffinity label [ 23].	bind
39708	4	9412	7	NULL	NULL	0	NULL	aN550	NULL		bind	NULL				GABAB receptor photoaffinity ligand	NULL				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_76_1_180_s_248	10719229	A chimeric receptor containing the ATD of the GABAB R1a subunit encompassing all of the ATD except the last 40 amino acids immediately upstream of the first TMD (termed aN550) bound a GABAB receptor photoaffinity ligand, while a construct fused 60 amino acids upstream of the first TMD (termed aN530) did not bind the photoaffinity label [ 23].	bind
39709	4	9412	7	NULL	NULL	0	NULL	chimeric receptor	NULL		contains	NULL					NULL		60 amino acids upstream of the first TMD		NULL		0	NULL	NULL	NULL	gw60_brainresmolbrainres_76_1_180_s_248	10719229	A chimeric receptor containing the ATD of the GABAB R1a subunit encompassing all of the ATD except the last 40 amino acids immediately upstream of the first TMD (termed aN550) bound a GABAB receptor photoaffinity ligand, while a construct fused 60 amino acids upstream of the first TMD (termed aN530) did not bind the photoaffinity label [ 23].	bind
39710	5	9412	7	NULL	NULL	0	NULL	chimeric receptor	NULL		is	NULL				aN530	NULL				NULL		0	NULL	NULL	NULL	gw60_brainresmolbrainres_76_1_180_s_248	10719229	A chimeric receptor containing the ATD of the GABAB R1a subunit encompassing all of the ATD except the last 40 amino acids immediately upstream of the first TMD (termed aN550) bound a GABAB receptor photoaffinity ligand, while a construct fused 60 amino acids upstream of the first TMD (termed aN530) did not bind the photoaffinity label [ 23].	bind
39711	6	9412	7	NULL	NULL	0	NULL	aN530	NULL		does not bind	NULL				GABAB receptor photoaffinity ligand	NULL				NULL		0	NULL	NULL	NULL	gw60_brainresmolbrainres_76_1_180_s_248	10719229	A chimeric receptor containing the ATD of the GABAB R1a subunit encompassing all of the ATD except the last 40 amino acids immediately upstream of the first TMD (termed aN550) bound a GABAB receptor photoaffinity ligand, while a construct fused 60 amino acids upstream of the first TMD (termed aN530) did not bind the photoaffinity label [ 23].	bind
39712	3	9412	7	NULL	NULL	0	NULL	chimeric receptor	NULL		is	NULL				aN550	NULL				NULL		0	NULL	NULL	NULL	gw60_brainresmolbrainres_76_1_180_s_248	10719229	A chimeric receptor containing the ATD of the GABAB R1a subunit encompassing all of the ATD except the last 40 amino acids immediately upstream of the first TMD (termed aN550) bound a GABAB receptor photoaffinity ligand, while a construct fused 60 amino acids upstream of the first TMD (termed aN530) did not bind the photoaffinity label [ 23].	bind
43077	1	9413	5	13	NULL	NULL	NULL	IP3R	GP		is substituted into			2318-2328		RyR	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_73_0_437_s_305	15189149	A chimeric RyR substitution of residues  2318-2328 of IP3R into RyR retained FKBP12 binding, although binding of native IP3R to FKBP12 could not be demonstrated.	bind
43082	2	9413	5	13	NULL	NULL	NULL	chimeric RyR	GP		bind					FKBP12	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_73_0_437_s_305	15189149	A chimeric RyR substitution of residues  2318-2328 of IP3R into RyR retained FKBP12 binding, although binding of native IP3R to FKBP12 could not be demonstrated.	bind
43083	3	9413	5	13	NULL	NULL	NULL	IP3R	GP	native	does not bind					FKBP12	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_73_0_437_s_305	15189149	A chimeric RyR substitution of residues  2318-2328 of IP3R into RyR retained FKBP12 binding, although binding of native IP3R to FKBP12 could not be demonstrated.	bind
39713	1	9413	7	NULL	NULL	0	NULL	chimeric RyR	NULL		substituted with	NULL				IP3R	NULL		 residues 2318-2328		NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_437_s_305	15189149	A chimeric RyR substitution of residues  2318-2328 of IP3R into RyR retained FKBP12 binding, although binding of native IP3R to FKBP12 could not be demonstrated.	bind
39714	2	9413	7	NULL	NULL	0	NULL	chimeric RyR	NULL		bind	NULL				FKBP12	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_437_s_305	15189149	A chimeric RyR substitution of residues  2318-2328 of IP3R into RyR retained FKBP12 binding, although binding of native IP3R to FKBP12 could not be demonstrated.	bind
39715	3	9413	7	NULL	NULL	0	NULL	IP3R	NULL	native	does not bind	NULL				FKBP12	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_437_s_305	15189149	A chimeric RyR substitution of residues  2318-2328 of IP3R into RyR retained FKBP12 binding, although binding of native IP3R to FKBP12 could not be demonstrated.	bind
43195	1	9414	5	13	NULL	NULL	NULL	chimeric STAT5 protein	GP		consists of					STAT5A	GP		first 545 amino acids		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_33936_s_105	9852045	A chimeric STAT5 protein containing the first 545 amino acids of STAT5A and the COOH terminus of STAT5B (AB) did not bind to the APRE probe behaving like STAT5A ( lanes 2 and  8), and the complementary chimera with the NH2-terminal 545 amino acids of STAT5B fused to the COOH terminus of STAT5A (5BA) had the recognition property of STAT5B, that is, it bound well to APRE probe ( lanes 4 and  6).	bind
43196	2	9414	5	13	NULL	NULL	NULL	chimeric STAT5 protein	GP		consists of					STAT5B	GP		COOH terminus		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_33936_s_105	9852045	A chimeric STAT5 protein containing the first 545 amino acids of STAT5A and the COOH terminus of STAT5B (AB) did not bind to the APRE probe behaving like STAT5A ( lanes 2 and  8), and the complementary chimera with the NH2-terminal 545 amino acids of STAT5B fused to the COOH terminus of STAT5A (5BA) had the recognition property of STAT5B, that is, it bound well to APRE probe ( lanes 4 and  6).	bind
43197	3	9414	5	13	NULL	NULL	NULL	APRE probe	GP		behave like					STAT5A	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_33936_s_105	9852045	A chimeric STAT5 protein containing the first 545 amino acids of STAT5A and the COOH terminus of STAT5B (AB) did not bind to the APRE probe behaving like STAT5A ( lanes 2 and  8), and the complementary chimera with the NH2-terminal 545 amino acids of STAT5B fused to the COOH terminus of STAT5A (5BA) had the recognition property of STAT5B, that is, it bound well to APRE probe ( lanes 4 and  6).	bind
43198	4	9414	5	13	NULL	NULL	NULL	statement 1	GP		does not bind					statement 3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_33936_s_105	9852045	A chimeric STAT5 protein containing the first 545 amino acids of STAT5A and the COOH terminus of STAT5B (AB) did not bind to the APRE probe behaving like STAT5A ( lanes 2 and  8), and the complementary chimera with the NH2-terminal 545 amino acids of STAT5B fused to the COOH terminus of STAT5A (5BA) had the recognition property of STAT5B, that is, it bound well to APRE probe ( lanes 4 and  6).	bind
43199	5	9414	5	13	NULL	NULL	NULL	statement 2	GP		does not bind					statement 3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_33936_s_105	9852045	A chimeric STAT5 protein containing the first 545 amino acids of STAT5A and the COOH terminus of STAT5B (AB) did not bind to the APRE probe behaving like STAT5A ( lanes 2 and  8), and the complementary chimera with the NH2-terminal 545 amino acids of STAT5B fused to the COOH terminus of STAT5A (5BA) had the recognition property of STAT5B, that is, it bound well to APRE probe ( lanes 4 and  6).	bind
43200	6	9414	5	13	NULL	NULL	NULL	STAT5B	GP		fused to			NH2-terminal 545 amino acids		STAT5A	GP		COOH terminus		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_33936_s_105	9852045	A chimeric STAT5 protein containing the first 545 amino acids of STAT5A and the COOH terminus of STAT5B (AB) did not bind to the APRE probe behaving like STAT5A ( lanes 2 and  8), and the complementary chimera with the NH2-terminal 545 amino acids of STAT5B fused to the COOH terminus of STAT5A (5BA) had the recognition property of STAT5B, that is, it bound well to APRE probe ( lanes 4 and  6).	bind
43201	7	9414	5	13	NULL	NULL	NULL	statement 6	GP		is					complementary chimera	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_33936_s_105	9852045	A chimeric STAT5 protein containing the first 545 amino acids of STAT5A and the COOH terminus of STAT5B (AB) did not bind to the APRE probe behaving like STAT5A ( lanes 2 and  8), and the complementary chimera with the NH2-terminal 545 amino acids of STAT5B fused to the COOH terminus of STAT5A (5BA) had the recognition property of STAT5B, that is, it bound well to APRE probe ( lanes 4 and  6).	bind
43202	8	9414	5	13	NULL	NULL	NULL	statement 7	GP		contains					STAT5B	GP	recognition property of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_33936_s_105	9852045	A chimeric STAT5 protein containing the first 545 amino acids of STAT5A and the COOH terminus of STAT5B (AB) did not bind to the APRE probe behaving like STAT5A ( lanes 2 and  8), and the complementary chimera with the NH2-terminal 545 amino acids of STAT5B fused to the COOH terminus of STAT5A (5BA) had the recognition property of STAT5B, that is, it bound well to APRE probe ( lanes 4 and  6).	bind
43203	9	9414	5	13	NULL	NULL	NULL	statement 7	GP		bind					APRE probe	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_33936_s_105	9852045	A chimeric STAT5 protein containing the first 545 amino acids of STAT5A and the COOH terminus of STAT5B (AB) did not bind to the APRE probe behaving like STAT5A ( lanes 2 and  8), and the complementary chimera with the NH2-terminal 545 amino acids of STAT5B fused to the COOH terminus of STAT5A (5BA) had the recognition property of STAT5B, that is, it bound well to APRE probe ( lanes 4 and  6).	bind
39716	1	9414	7	NULL	NULL	0	NULL	chimeric STAT5 protein 	NULL		contains	NULL				STAT5A	NULL		first 545 amino acids 		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_33936_s_105	9852045	A chimeric STAT5 protein containing the first 545 amino acids of STAT5A and the COOH terminus of STAT5B (AB) did not bind to the APRE probe behaving like STAT5A ( lanes 2 and  8), and the complementary chimera with the NH2-terminal 545 amino acids of STAT5B fused to the COOH terminus of STAT5A (5BA) had the recognition property of STAT5B, that is, it bound well to APRE probe ( lanes 4 and  6).	bind
39717	2	9414	7	NULL	NULL	0	NULL	chimeric STAT5 protein	NULL		contains	NULL				STAT5B	NULL		COOH terminus of		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_51_33936_s_105	9852045	A chimeric STAT5 protein containing the first 545 amino acids of STAT5A and the COOH terminus of STAT5B (AB) did not bind to the APRE probe behaving like STAT5A ( lanes 2 and  8), and the complementary chimera with the NH2-terminal 545 amino acids of STAT5B fused to the COOH terminus of STAT5A (5BA) had the recognition property of STAT5B, that is, it bound well to APRE probe ( lanes 4 and  6).	bind
39718	3	9414	7	NULL	NULL	0	NULL	chimeric STAT5 protein	NULL		does not bind	NULL				APRE probe	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_51_33936_s_105	9852045	A chimeric STAT5 protein containing the first 545 amino acids of STAT5A and the COOH terminus of STAT5B (AB) did not bind to the APRE probe behaving like STAT5A ( lanes 2 and  8), and the complementary chimera with the NH2-terminal 545 amino acids of STAT5B fused to the COOH terminus of STAT5A (5BA) had the recognition property of STAT5B, that is, it bound well to APRE probe ( lanes 4 and  6).	bind
39719	4	9414	7	NULL	NULL	0	NULL	chimeric STAT5 protein	NULL		behave like	NULL				STAT5A	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_51_33936_s_105	9852045	A chimeric STAT5 protein containing the first 545 amino acids of STAT5A and the COOH terminus of STAT5B (AB) did not bind to the APRE probe behaving like STAT5A ( lanes 2 and  8), and the complementary chimera with the NH2-terminal 545 amino acids of STAT5B fused to the COOH terminus of STAT5A (5BA) had the recognition property of STAT5B, that is, it bound well to APRE probe ( lanes 4 and  6).	bind
39720	5	9414	7	NULL	NULL	0	NULL	chimera	NULL		contains	NULL				STAT5B	NULL		NH2-terminal 545 amino acids of 		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_51_33936_s_105	9852045	A chimeric STAT5 protein containing the first 545 amino acids of STAT5A and the COOH terminus of STAT5B (AB) did not bind to the APRE probe behaving like STAT5A ( lanes 2 and  8), and the complementary chimera with the NH2-terminal 545 amino acids of STAT5B fused to the COOH terminus of STAT5A (5BA) had the recognition property of STAT5B, that is, it bound well to APRE probe ( lanes 4 and  6).	bind
39721	6	9414	7	NULL	NULL	0	NULL	chimera	NULL		contains	NULL				STAT5A	NULL		COOH terminus of		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_51_33936_s_105	9852045	A chimeric STAT5 protein containing the first 545 amino acids of STAT5A and the COOH terminus of STAT5B (AB) did not bind to the APRE probe behaving like STAT5A ( lanes 2 and  8), and the complementary chimera with the NH2-terminal 545 amino acids of STAT5B fused to the COOH terminus of STAT5A (5BA) had the recognition property of STAT5B, that is, it bound well to APRE probe ( lanes 4 and  6).	bind
39722	8	9414	7	NULL	NULL	0	NULL	chimera	NULL		bind	NULL				APRE probe	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_33936_s_105	9852045	A chimeric STAT5 protein containing the first 545 amino acids of STAT5A and the COOH terminus of STAT5B (AB) did not bind to the APRE probe behaving like STAT5A ( lanes 2 and  8), and the complementary chimera with the NH2-terminal 545 amino acids of STAT5B fused to the COOH terminus of STAT5A (5BA) had the recognition property of STAT5B, that is, it bound well to APRE probe ( lanes 4 and  6).	bind
39723	7	9414	7	NULL	NULL	0	NULL	chimera	NULL		behave like	NULL				STAT5B	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_51_33936_s_105	9852045	A chimeric STAT5 protein containing the first 545 amino acids of STAT5A and the COOH terminus of STAT5B (AB) did not bind to the APRE probe behaving like STAT5A ( lanes 2 and  8), and the complementary chimera with the NH2-terminal 545 amino acids of STAT5B fused to the COOH terminus of STAT5A (5BA) had the recognition property of STAT5B, that is, it bound well to APRE probe ( lanes 4 and  6).	bind
43204	1	9415	5	13	NULL	NULL	NULL	chimeric tetramer	GP		is composed of					ubiquitins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34983_s_8	9857030	A chimeric tetramer composed of three ubiquitins and one histidine-tagged NEDD8 binds to the 26 S proteasome with an affinity similar to that of tetraubiquitin.	bind
43205	2	9415	5	13	NULL	NULL	NULL	chimeric tetramer	GP		is composed of					NEDD8	GP	histidine-tagged			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34983_s_8	9857030	A chimeric tetramer composed of three ubiquitins and one histidine-tagged NEDD8 binds to the 26 S proteasome with an affinity similar to that of tetraubiquitin.	bind
43206	3	9415	5	13	NULL	NULL	NULL	statement 1	GP		bind					26 S proteasome	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34983_s_8	9857030	A chimeric tetramer composed of three ubiquitins and one histidine-tagged NEDD8 binds to the 26 S proteasome with an affinity similar to that of tetraubiquitin.	bind
43207	4	9415	5	13	NULL	NULL	NULL	statement 2	GP		bind					26 S proteasome	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34983_s_8	9857030	A chimeric tetramer composed of three ubiquitins and one histidine-tagged NEDD8 binds to the 26 S proteasome with an affinity similar to that of tetraubiquitin.	bind
43208	5	9415	5	13	NULL	NULL	NULL	statement 1	GP		bind					tetraubiquitin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34983_s_8	9857030	A chimeric tetramer composed of three ubiquitins and one histidine-tagged NEDD8 binds to the 26 S proteasome with an affinity similar to that of tetraubiquitin.	bind
43209	6	9415	5	13	NULL	NULL	NULL	statement 2	GP		bind					tetraubiquitin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34983_s_8	9857030	A chimeric tetramer composed of three ubiquitins and one histidine-tagged NEDD8 binds to the 26 S proteasome with an affinity similar to that of tetraubiquitin.	bind
43210	7	9415	5	13	NULL	NULL	NULL	statement 3	Process		similar affinity to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34983_s_8	9857030	A chimeric tetramer composed of three ubiquitins and one histidine-tagged NEDD8 binds to the 26 S proteasome with an affinity similar to that of tetraubiquitin.	bind
43211	8	9415	5	13	NULL	NULL	NULL	statement 4	Process		similar affinity to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34983_s_8	9857030	A chimeric tetramer composed of three ubiquitins and one histidine-tagged NEDD8 binds to the 26 S proteasome with an affinity similar to that of tetraubiquitin.	bind
39725	1	9415	7	10	NULL	0	NULL	chimeric tetramer	NULL		is composed of	NULL				NEDD8	NULL	histidine tagged			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34983_s_8	9857030	A chimeric tetramer composed of three ubiquitins and one histidine-tagged NEDD8 binds to the 26 S proteasome with an affinity similar to that of tetraubiquitin.	bind
39726	4	9415	7	NULL	NULL	0	NULL	statement 3	NULL		binds to	NULL				26 S proteasome	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34983_s_8	9857030	A chimeric tetramer composed of three ubiquitins and one histidine-tagged NEDD8 binds to the 26 S proteasome with an affinity similar to that of tetraubiquitin.	bind
39727	5	9415	7	NULL	NULL	0	NULL	tetraubiquitin	NULL		bind	NULL				26 S proteasome	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34983_s_8	9857030	A chimeric tetramer composed of three ubiquitins and one histidine-tagged NEDD8 binds to the 26 S proteasome with an affinity similar to that of tetraubiquitin.	bind
46959	2	9415	7	NULL	NULL	0	NULL	chimeric tetramer	NULL		is composed of	NULL				three ubiquitins 	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34983_s_8	9857030	A chimeric tetramer composed of three ubiquitins and one histidine-tagged NEDD8 binds to the 26 S proteasome with an affinity similar to that of tetraubiquitin.	bind
46960	3	9415	7	NULL	NULL	0	NULL	statement 1	NULL		occur along with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_52_34983_s_8	9857030	A chimeric tetramer composed of three ubiquitins and one histidine-tagged NEDD8 binds to the 26 S proteasome with an affinity similar to that of tetraubiquitin.	bind
46961	6	9415	7	NULL	NULL	0	NULL	statement 4	NULL	affinity of	is similar to	NULL				statement 5	NULL	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34983_s_8	9857030	A chimeric tetramer composed of three ubiquitins and one histidine-tagged NEDD8 binds to the 26 S proteasome with an affinity similar to that of tetraubiquitin.	bind
41065	1	9416	5	13	NULL	NULL	NULL	PAX3-FKHR	GP		is a type of					chimeric transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_30_23259_s_23	10770948	A chimeric transcription factor PAX3-FKHR, produced by this t(2;13)(q35;q14) chromosomal translocation in alveolar rhabdomyosarcoma binds to the NCAM promoter through its Pax3 homeodomain recognition helix.	bind
41066	2	9416	5	13	NULL	NULL	NULL	PAX3-FKHR	GP		produced by							chromosomal translocation of		t(2;13)(q35;q14)	NULL	alveolar rhabdomyosarcoma 	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_30_23259_s_23	10770948	A chimeric transcription factor PAX3-FKHR, produced by this t(2;13)(q35;q14) chromosomal translocation in alveolar rhabdomyosarcoma binds to the NCAM promoter through its Pax3 homeodomain recognition helix.	bind
41067	3	9416	5	13	NULL	NULL	NULL	PAX3-FKHR	GP		bind			Pax3 homeodomain recognition helix		NCAM 	NucleicAcid			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_30_23259_s_23	10770948	A chimeric transcription factor PAX3-FKHR, produced by this t(2;13)(q35;q14) chromosomal translocation in alveolar rhabdomyosarcoma binds to the NCAM promoter through its Pax3 homeodomain recognition helix.	bind
39728	1	9416	7	10	NULL	0	NULL	PAX3-FKHR	NULL		is produced by	NULL				t(2;13)(q35;q14) 	NULL	chromosomal translocation of			NULL	alveolar rhabdomyosarcoma	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_30_23259_s_23	10770948	A chimeric transcription factor PAX3-FKHR, produced by this t(2;13)(q35;q14) chromosomal translocation in alveolar rhabdomyosarcoma binds to the NCAM promoter through its Pax3 homeodomain recognition helix.	bind
39729	2	9416	7	NULL	NULL	0	NULL	chimeric transcription factor PAX3-FKHR	NULL		binds to	NULL		Pax3 homeodomain recognition helix		NCAM	NULL			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_30_23259_s_23	10770948	A chimeric transcription factor PAX3-FKHR, produced by this t(2;13)(q35;q14) chromosomal translocation in alveolar rhabdomyosarcoma binds to the NCAM promoter through its Pax3 homeodomain recognition helix.	bind
46830	3	9416	7	10	NULL	0	NULL	PAX3-FKHR	NULL		is a type of 	NULL				chimeric transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_30_23259_s_23	10770948	A chimeric transcription factor PAX3-FKHR, produced by this t(2;13)(q35;q14) chromosomal translocation in alveolar rhabdomyosarcoma binds to the NCAM promoter through its Pax3 homeodomain recognition helix.	bind
41069	1	9417	5	13	NULL	NULL	NULL	chimeric virus	Organism		does not bind					Z-DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_12_6974_s_5	12777633	A chimeric virus incorporating a  related protein that does not bind Z-DNA is not pathogenic, but a mutation  that creates Z-DNA binding makes a lethal virus.	bind
41071	2	9417	5	13	NULL	NULL	NULL	statement 1	Organism		is not					pathogenic	Organism				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_12_6974_s_5	12777633	A chimeric virus incorporating a  related protein that does not bind Z-DNA is not pathogenic, but a mutation  that creates Z-DNA binding makes a lethal virus.	bind
41072	3	9417	5	13	NULL	NULL	NULL	chimeric virus	Organism	mutant	bind					Z-DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_12_6974_s_5	12777633	A chimeric virus incorporating a  related protein that does not bind Z-DNA is not pathogenic, but a mutation  that creates Z-DNA binding makes a lethal virus.	bind
41073	4	9417	5	13	NULL	NULL	NULL	statement 3	Organism		is a type of 					lethal virus	Organism				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_12_6974_s_5	12777633	A chimeric virus incorporating a  related protein that does not bind Z-DNA is not pathogenic, but a mutation  that creates Z-DNA binding makes a lethal virus.	bind
39730	1	9417	7	NULL	NULL	0	NULL	chimeric virus	NULL		does not bind	NULL				Z-DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_100_12_6974_s_5	12777633	A chimeric virus incorporating a  related protein that does not bind Z-DNA is not pathogenic, but a mutation  that creates Z-DNA binding makes a lethal virus.	bind
39731	2	9417	7	NULL	NULL	0	NULL	statement 1	NULL		is not	NULL				pathogenic	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_100_12_6974_s_5	12777633	A chimeric virus incorporating a  related protein that does not bind Z-DNA is not pathogenic, but a mutation  that creates Z-DNA binding makes a lethal virus.	bind
39732	3	9417	7	NULL	NULL	0	NULL	chimeric virus	NULL	mutated	binds	NULL				Z-DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_100_12_6974_s_5	12777633	A chimeric virus incorporating a  related protein that does not bind Z-DNA is not pathogenic, but a mutation  that creates Z-DNA binding makes a lethal virus.	bind
39733	4	9417	7	NULL	NULL	0	NULL	statement 3	NULL		is a type of	NULL				lethal virus	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_100_12_6974_s_5	12777633	A chimeric virus incorporating a  related protein that does not bind Z-DNA is not pathogenic, but a mutation  that creates Z-DNA binding makes a lethal virus.	bind
41074	1	9418	5	13	NULL	NULL	NULL	(IRS) 2/FRS3 adapter	GP		is a type of					chimerical insulin receptor substrate	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1763_4_366_s_191	16697063	A chimerical insulin receptor substrate (IRS) 2/FRS3 adapter supports insulin-dependent  MAPK/ERK activation and neuritogenesis and is dependent upon the integrity of the  Grb2 and Shp2 binding sites of FRS3	bind
41075	2	9418	5	13	NULL	NULL	NULL	(IRS) 2/FRS3 adapter	GP		supports					MAPK/ERK	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1763_4_366_s_191	16697063	A chimerical insulin receptor substrate (IRS) 2/FRS3 adapter supports insulin-dependent  MAPK/ERK activation and neuritogenesis and is dependent upon the integrity of the  Grb2 and Shp2 binding sites of FRS3	bind
41076	3	9418	5	13	NULL	NULL	NULL	MAPK/ERK	GP	activation of	is dependent on					insulin	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1763_4_366_s_191	16697063	A chimerical insulin receptor substrate (IRS) 2/FRS3 adapter supports insulin-dependent  MAPK/ERK activation and neuritogenesis and is dependent upon the integrity of the  Grb2 and Shp2 binding sites of FRS3	bind
41078	4	9418	5	13	NULL	NULL	NULL	(IRS) 2/FRS3 adapter	GP		supports					neuritogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1763_4_366_s_191	16697063	A chimerical insulin receptor substrate (IRS) 2/FRS3 adapter supports insulin-dependent  MAPK/ERK activation and neuritogenesis and is dependent upon the integrity of the  Grb2 and Shp2 binding sites of FRS3	bind
41079	5	9418	5	13	NULL	NULL	NULL	(IRS) 2/FRS3 adapter	GP		is dependent on					FRS3	GP	integrity of	Shp2 binding sites		NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1763_4_366_s_191	16697063	A chimerical insulin receptor substrate (IRS) 2/FRS3 adapter supports insulin-dependent  MAPK/ERK activation and neuritogenesis and is dependent upon the integrity of the  Grb2 and Shp2 binding sites of FRS3	bind
41081	6	9418	5	13	NULL	NULL	NULL	(IRS) 2/FRS3 adapter	GP		is dependent on					FRS3	GP	integrity of	Grb2 binding sites		NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1763_4_366_s_191	16697063	A chimerical insulin receptor substrate (IRS) 2/FRS3 adapter supports insulin-dependent  MAPK/ERK activation and neuritogenesis and is dependent upon the integrity of the  Grb2 and Shp2 binding sites of FRS3	bind
39734	1	9418	7	NULL	NULL	0	NULL	MAPK/ERK 	NULL	activation of	depends on	NULL				insulin	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1763_4_366_s_191	16697063	A chimerical insulin receptor substrate (IRS) 2/FRS3 adapter supports insulin-dependent  MAPK/ERK activation and neuritogenesis and is dependent upon the integrity of the  Grb2 and Shp2 binding sites of FRS3	bind
39735	2	9418	7	10	NULL	0	NULL	(IRS) 2/FRS3			supports					statement 1					NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1763_4_366_s_191	16697063	A chimerical insulin receptor substrate (IRS) 2/FRS3 adapter supports insulin-dependent  MAPK/ERK activation and neuritogenesis and is dependent upon the integrity of the  Grb2 and Shp2 binding sites of FRS3	bind
39736	3	9418	7	NULL	NULL	0	NULL	neuritogenesis	NULL		depends on	NULL				insulin	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1763_4_366_s_191	16697063	A chimerical insulin receptor substrate (IRS) 2/FRS3 adapter supports insulin-dependent  MAPK/ERK activation and neuritogenesis and is dependent upon the integrity of the  Grb2 and Shp2 binding sites of FRS3	bind
39737	4	9418	7	10	NULL	0	NULL	(IRS) 2/FRS3			supports					statement 3					NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1763_4_366_s_191	16697063	A chimerical insulin receptor substrate (IRS) 2/FRS3 adapter supports insulin-dependent  MAPK/ERK activation and neuritogenesis and is dependent upon the integrity of the  Grb2 and Shp2 binding sites of FRS3	bind
39738	5	9418	7	10	NULL	0	NULL	(IRS) 2/FRS3			is dependent on					FRS3		integrity of	Grb2 binding site		NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1763_4_366_s_191	16697063	A chimerical insulin receptor substrate (IRS) 2/FRS3 adapter supports insulin-dependent  MAPK/ERK activation and neuritogenesis and is dependent upon the integrity of the  Grb2 and Shp2 binding sites of FRS3	bind
39739	6	9418	7	10	NULL	0	NULL	(IRS) 2/FRS3			is dependent on					FRS3		integrity of	Shp2 binding site		NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1763_4_366_s_191	16697063	A chimerical insulin receptor substrate (IRS) 2/FRS3 adapter supports insulin-dependent  MAPK/ERK activation and neuritogenesis and is dependent upon the integrity of the  Grb2 and Shp2 binding sites of FRS3	bind
56711	7	9418	7	10	NULL	0	NULL	(IRS) 2/FRS3			is a type of					chimeric insulin receptor substrate					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1763_4_366_s_191	16697063	A chimerical insulin receptor substrate (IRS) 2/FRS3 adapter supports insulin-dependent  MAPK/ERK activation and neuritogenesis and is dependent upon the integrity of the  Grb2 and Shp2 binding sites of FRS3	bind
41082	1	9419	5	13	NULL	NULL	NULL	CBP	GP		bind					IL-10	NucleicAcid	proximal		promoter	NULL	in situ in LPS-stimulated primary macrophages	NULL	NULL	NULL	NULL	gw70_jbiolchem_281_36_26041_s_218	16835236	A ChIP analysis was performed on stimulated cells, and this assay verified that CBP binds to the proximal IL-10 promoter  in situ in LPS-stimulated primary macrophages ( Fig. 6 C), although the kinetics of CBP association appeared to be slightly different from that of p50 ( Fig. 6 C).	bind
39742	1	9419	7	NULL	NULL	0	NULL	CBP	NULL		binds to	NULL				IL-10	NULL	proximal		promoter	NULL	in situ in LPS-stimulated primary macrophages	0	NULL	NULL	NULL	gw70_jbiolchem_281_36_26041_s_218	16835236	A ChIP analysis was performed on stimulated cells, and this assay verified that CBP binds to the proximal IL-10 promoter  in situ in LPS-stimulated primary macrophages ( Fig. 6 C), although the kinetics of CBP association appeared to be slightly different from that of p50 ( Fig. 6 C).	bind
41050	1	9420	5	13	NULL	NULL	NULL	SREBP-1	GP		bind					LGK	NucleicAcid			SREs of promoter	NULL	primary hepatocytes	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_29_30823_s_280	15123649	A ChIP assay using primary hepatocytes showed the increased binding of SREBP-1 to SREs of LGK promoter.	bind
39745	1	9420	7	NULL	NULL	0	NULL	SREBP-1 	NULL		bind	NULL				LGK	NULL			SREs in the promoter	NULL	primary hepatocytes	0	NULL	NULL	NULL	gw70_jbiolchem_279_29_30823_s_280	15123649	A ChIP assay using primary hepatocytes showed the increased binding of SREBP-1 to SREs of LGK promoter.	bind
41051	1	9421	5	13	NULL	NULL	NULL	Smad4	GP		bind					Ihh gene 	GP			GC-rich motifs within -285/-123 region	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_18544_s_162	14981086	A ChIP assay was carried out to confirm that Smad4 binds to GC-rich motifs within the -285/-123 region of the  Ihh gene upon BMP7 stimulation  in vivo.	bind
41052	2	9421	5	13	NULL	NULL	NULL	BMP7	GP	stimulation of	leads to					statement 1	Process				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_18544_s_162	14981086	A ChIP assay was carried out to confirm that Smad4 binds to GC-rich motifs within the -285/-123 region of the  Ihh gene upon BMP7 stimulation  in vivo.	bind
39746	1	9421	7	NULL	NULL	0	NULL	Smad4 	NULL		binds to	NULL				Ihh gene	NULL			GC-rich motifs within the -285/-123 region	NULL	in vivo	0	NULL	NULL	NULL	gw70_jbiolchem_279_18_18544_s_162	14981086	A ChIP assay was carried out to confirm that Smad4 binds to GC-rich motifs within the -285/-123 region of the  Ihh gene upon BMP7 stimulation  in vivo.	bind
39747	2	9421	7	NULL	NULL	0	NULL	statement 1	NULL		occurs upon	NULL				BMP7 	NULL	stimulation of			NULL	in vivo	0	NULL	NULL	NULL	gw70_jbiolchem_279_18_18544_s_162	14981086	A ChIP assay was carried out to confirm that Smad4 binds to GC-rich motifs within the -285/-123 region of the  Ihh gene upon BMP7 stimulation  in vivo.	bind
41053	1	9423	5	13	NULL	NULL	NULL	cholera toxin	Chemical		bind			B-subunit variant		ganglioside GM1	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_71_3_1527_s_583	12595472	A cholera toxin B-subunit variant that binds ganglioside GM1 but fails to induce toxicity.	bind
41054	2	9423	5	13	NULL	NULL	NULL	statement 1	Process		does not induce					toxicity	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_71_3_1527_s_583	12595472	A cholera toxin B-subunit variant that binds ganglioside GM1 but fails to induce toxicity.	bind
39748	1	9423	7	NULL	NULL	0	NULL	cholera toxin 	NULL		binds	NULL		B-subunit variant		ganglioside GM1	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_71_3_1527_s_583	12595472	A cholera toxin B-subunit variant that binds ganglioside GM1 but fails to induce toxicity.	bind
39749	2	9423	7	NULL	NULL	0	NULL	statement 1	NULL		fails to induce	NULL				toxicity	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_71_3_1527_s_583	12595472	A cholera toxin B-subunit variant that binds ganglioside GM1 but fails to induce toxicity.	bind
41085	1	9424	5	13	NULL	NULL	NULL	mcl-1	GP		bind									SIE motif of promoter	NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_mol-cell-biol_23_6_12612065_s_5	12612065	A chromatin immunoprecipitation  assay further confirmed that PU.1 binds to the mcl-1 promoter region containing  the SIE motif in vivo.	bind
39750	1	9424	7	10	NULL	0	NULL	 PU.1			binds to					 mcl-1				 SIE motif of promoter	NULL	in vivo	NULL	NULL	NULL	NULL	abs-batch0650-0679_mol-cell-biol_23_6_12612065_s_5	12612065	A chromatin immunoprecipitation  assay further confirmed that PU.1 binds to the mcl-1 promoter region containing  the SIE motif in vivo.	bind
41088	1	9426	5	13	NULL	NULL	NULL	Mitf	GP		bind					p21 Cip1	NucleicAcid			promoter	NULL	mel melanoma cells	NULL	NULL	NULL	NULL	gw70_nature_433_7027_764_s_49	15716956	A chromatin immunoprecipitation assay (ChIP) from 501mel  melanoma cells, which express both Mitf and p21Cip1, or melan-a melanocytes, using an anti-Mitf antibody and polymerase chain reaction  (PCR) primers spanning the  p21 Cip1 E2 element confirmed Mitf binding to the  p21 Cip1 promoter  in vivo ( Fig. 2e).	bind
41089	2	9426	5	13	NULL	NULL	NULL	mel melanoma cells	Cell		express					Mitf	GP				NULL		NULL	NULL	NULL	NULL	gw70_nature_433_7027_764_s_49	15716956	A chromatin immunoprecipitation assay (ChIP) from 501mel  melanoma cells, which express both Mitf and p21Cip1, or melan-a melanocytes, using an anti-Mitf antibody and polymerase chain reaction  (PCR) primers spanning the  p21 Cip1 E2 element confirmed Mitf binding to the  p21 Cip1 promoter  in vivo ( Fig. 2e).	bind
41090	3	9426	5	13	NULL	NULL	NULL	Mitf	GP		bind					p21 Cip1	NucleicAcid			promoter	NULL	melan-a melanocytes	NULL	NULL	NULL	NULL	gw70_nature_433_7027_764_s_49	15716956	A chromatin immunoprecipitation assay (ChIP) from 501mel  melanoma cells, which express both Mitf and p21Cip1, or melan-a melanocytes, using an anti-Mitf antibody and polymerase chain reaction  (PCR) primers spanning the  p21 Cip1 E2 element confirmed Mitf binding to the  p21 Cip1 promoter  in vivo ( Fig. 2e).	bind
41091	4	9426	5	13	NULL	NULL	NULL	mel melanoma cells	Cell		express					p21Cip1	GP				NULL		NULL	NULL	NULL	NULL	gw70_nature_433_7027_764_s_49	15716956	A chromatin immunoprecipitation assay (ChIP) from 501mel  melanoma cells, which express both Mitf and p21Cip1, or melan-a melanocytes, using an anti-Mitf antibody and polymerase chain reaction  (PCR) primers spanning the  p21 Cip1 E2 element confirmed Mitf binding to the  p21 Cip1 promoter  in vivo ( Fig. 2e).	bind
39755	1	9426	7	NULL	NULL	0	NULL	Mitf	NULL		bind	NULL				p21 Cip1	NULL			promoter	NULL	in vivo melanoma cells	NULL	NULL	NULL	NULL	gw70_nature_433_7027_764_s_49	15716956	A chromatin immunoprecipitation assay (ChIP) from 501mel  melanoma cells, which express both Mitf and p21Cip1, or melan-a melanocytes, using an anti-Mitf antibody and polymerase chain reaction  (PCR) primers spanning the  p21 Cip1 E2 element confirmed Mitf binding to the  p21 Cip1 promoter  in vivo ( Fig. 2e).	bind
39756	2	9426	7	NULL	NULL	0	NULL	melanoma cells	NULL		express	NULL				Mitf 	NULL				NULL		0	NULL	NULL	NULL	gw70_nature_433_7027_764_s_49	15716956	A chromatin immunoprecipitation assay (ChIP) from 501mel  melanoma cells, which express both Mitf and p21Cip1, or melan-a melanocytes, using an anti-Mitf antibody and polymerase chain reaction  (PCR) primers spanning the  p21 Cip1 E2 element confirmed Mitf binding to the  p21 Cip1 promoter  in vivo ( Fig. 2e).	bind
39757	3	9426	7	NULL	NULL	0	NULL	melanoma cells	NULL		express	NULL				p21Cip1	NULL				NULL		0	NULL	NULL	NULL	gw70_nature_433_7027_764_s_49	15716956	A chromatin immunoprecipitation assay (ChIP) from 501mel  melanoma cells, which express both Mitf and p21Cip1, or melan-a melanocytes, using an anti-Mitf antibody and polymerase chain reaction  (PCR) primers spanning the  p21 Cip1 E2 element confirmed Mitf binding to the  p21 Cip1 promoter  in vivo ( Fig. 2e).	bind
39758	4	9426	7	NULL	NULL	0	NULL	Mitf	NULL		bind	NULL				p21 Cip1	NULL			promoter	NULL	in vivo  melan-a melanocytes	0	NULL	NULL	NULL	gw70_nature_433_7027_764_s_49	15716956	A chromatin immunoprecipitation assay (ChIP) from 501mel  melanoma cells, which express both Mitf and p21Cip1, or melan-a melanocytes, using an anti-Mitf antibody and polymerase chain reaction  (PCR) primers spanning the  p21 Cip1 E2 element confirmed Mitf binding to the  p21 Cip1 promoter  in vivo ( Fig. 2e).	bind
41092	1	9427	5	13	NULL	NULL	NULL	Rgt1	GP		bind					HXT1	GP			promoter	NULL	cells grown on galactose	NULL	NULL	NULL	NULL	gw70_jbiolchem_281_36_26144_s_115	16844691	A chromatin immunoprecipitation assay confirms that Rgt1 binds to the  HXT1 promoter in cells grown on galactose but not glucose ( Fig. 6 A).	bind
41095	2	9427	5	13	NULL	NULL	NULL	Rgt1	GP		does not bind					HXT1	GP			promoter	NULL	cells grown on glucose	NULL	NULL	NULL	NULL	gw70_jbiolchem_281_36_26144_s_115	16844691	A chromatin immunoprecipitation assay confirms that Rgt1 binds to the  HXT1 promoter in cells grown on galactose but not glucose ( Fig. 6 A).	bind
39759	1	9427	7	NULL	NULL	0	NULL	Rgt1	NULL		binds to	NULL				HXT1	NULL			promoter	NULL	cells grown on galactose 	0	NULL	NULL	NULL	gw70_jbiolchem_281_36_26144_s_115	16844691	A chromatin immunoprecipitation assay confirms that Rgt1 binds to the  HXT1 promoter in cells grown on galactose but not glucose ( Fig. 6 A).	bind
39760	2	9427	7	NULL	NULL	0	NULL	Rgt1	NULL		does not bind	NULL				HXT1	NULL			promoter	NULL	cells grown on glucose	0	NULL	NULL	NULL	gw70_jbiolchem_281_36_26144_s_115	16844691	A chromatin immunoprecipitation assay confirms that Rgt1 binds to the  HXT1 promoter in cells grown on galactose but not glucose ( Fig. 6 A).	bind
41096	1	9428	5	13	NULL	NULL	NULL	mcl-1	NucleicAcid		contains				promoter					SIE motif	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_6_1896_s_5	12612065	A chromatin immunoprecipitation assay further confirmed that PU.1 binds to the  mcl-1 promoter region containing the SIE motif in vivo.	bind
41097	2	9428	5	NULL	NULL	0	NULL	PU.1	NULL		bind	NULL				statement 1	NULL				NULL	in vivo	0	NULL	NULL	NULL	gw60_molcellbiol_23_6_1896_s_5	12612065	A chromatin immunoprecipitation assay further confirmed that PU.1 binds to the  mcl-1 promoter region containing the SIE motif in vivo.	bind
41098	1	9429	5	13	NULL	NULL	NULL	E2F-1	GP		bind					Apaf-1	NucleicAcid			promoter	NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_j-biol-chem_277_42_12149244_s_8	12149244	A chromatin immunoprecipitation assay revealed that  E2F-1 bound to Apaf-1 promoter upon E2F-1 overexpression, suggesting that  Apaf-1 is under transcriptional regulation of E2F-1.	bind
41100	2	9429	5	13	NULL	NULL	NULL	E2F-1	GP	overexpression of	leads to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_j-biol-chem_277_42_12149244_s_8	12149244	A chromatin immunoprecipitation assay revealed that  E2F-1 bound to Apaf-1 promoter upon E2F-1 overexpression, suggesting that  Apaf-1 is under transcriptional regulation of E2F-1.	bind
41102	3	9429	5	13	NULL	NULL	NULL	E2F-1	GP		regulates		transcriptionally			Apaf-1	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_j-biol-chem_277_42_12149244_s_8	12149244	A chromatin immunoprecipitation assay revealed that  E2F-1 bound to Apaf-1 promoter upon E2F-1 overexpression, suggesting that  Apaf-1 is under transcriptional regulation of E2F-1.	bind
41103	4	9429	5	13	NULL	NULL	NULL	statement 1	Process		suggest					statement 3	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_j-biol-chem_277_42_12149244_s_8	12149244	A chromatin immunoprecipitation assay revealed that  E2F-1 bound to Apaf-1 promoter upon E2F-1 overexpression, suggesting that  Apaf-1 is under transcriptional regulation of E2F-1.	bind
39761	1	9429	7	NULL	NULL	0	NULL	E2F-1	NULL		bind	NULL				Apaf-1	NULL			promoter	NULL		0	NULL	NULL	NULL	abs-batch0570-0579_j-biol-chem_277_42_12149244_s_8	12149244	A chromatin immunoprecipitation assay revealed that  E2F-1 bound to Apaf-1 promoter upon E2F-1 overexpression, suggesting that  Apaf-1 is under transcriptional regulation of E2F-1.	bind
39762	2	9429	7	NULL	NULL	0	NULL	statement 1	NULL		occurs upon	NULL				E2F-1	NULL	overexpression of			NULL		0	NULL	NULL	NULL	abs-batch0570-0579_j-biol-chem_277_42_12149244_s_8	12149244	A chromatin immunoprecipitation assay revealed that  E2F-1 bound to Apaf-1 promoter upon E2F-1 overexpression, suggesting that  Apaf-1 is under transcriptional regulation of E2F-1.	bind
39763	3	9429	7	NULL	NULL	0	NULL	E2F-1	NULL		regulates	NULL				Apaf-1	NULL	transcription of			NULL		0	NULL	NULL	NULL	abs-batch0570-0579_j-biol-chem_277_42_12149244_s_8	12149244	A chromatin immunoprecipitation assay revealed that  E2F-1 bound to Apaf-1 promoter upon E2F-1 overexpression, suggesting that  Apaf-1 is under transcriptional regulation of E2F-1.	bind
39764	4	9429	7	NULL	NULL	0	NULL	statement 1	NULL		suggests	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	abs-batch0570-0579_j-biol-chem_277_42_12149244_s_8	12149244	A chromatin immunoprecipitation assay revealed that  E2F-1 bound to Apaf-1 promoter upon E2F-1 overexpression, suggesting that  Apaf-1 is under transcriptional regulation of E2F-1.	bind
41104	1	9430	5	13	NULL	NULL	NULL	SREBP-1	GP		bind					LGK	NucleicAcid			SREs of promoter	NULL	primary hepatocytes	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_29_30823_s_10	15123649	A chromatin immunoprecipitation assay using primary hepatocytes showed increased binding of SREBP-1 to SREs of the LGK promoter by insulin.	bind
41105	2	9430	5	13	NULL	NULL	NULL	insulin	GP		increase					statement 1	Process				NULL	primary hepatocytes	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_29_30823_s_10	15123649	A chromatin immunoprecipitation assay using primary hepatocytes showed increased binding of SREBP-1 to SREs of the LGK promoter by insulin.	bind
39765	1	9430	7	NULL	NULL	0	NULL	SREBP-1 	NULL		bind	NULL				LGK	NULL			SREs in the promoter	NULL	primary hepatocytes	0	NULL	NULL	NULL	gw70_jbiolchem_279_29_30823_s_10	15123649	A chromatin immunoprecipitation assay using primary hepatocytes showed increased binding of SREBP-1 to SREs of the LGK promoter by insulin.	bind
39766	2	9430	7	NULL	NULL	0	NULL	insulin	NULL		increase	NULL				statement 1	NULL				NULL	primary hepatocytes	0	NULL	NULL	NULL	gw70_jbiolchem_279_29_30823_s_10	15123649	A chromatin immunoprecipitation assay using primary hepatocytes showed increased binding of SREBP-1 to SREs of the LGK promoter by insulin.	bind
41106	1	9431	5	13	NULL	NULL	NULL	DNA fragments	NucleicAcid	Drosophila	bind					Engrailed protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_20_7097_s_220	15870192	A chromatin immunoprecipitation procedure also has been used to identify DNA binding sites; 203  Drosophila DNA fragments that bind the Engrailed protein were localized in intergenic (53%) or intronic (47%) regions ( ).	bind
41107	2	9431	5	13	NULL	NULL	NULL	statement 1	GP		is localized in									intergenic regions	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_20_7097_s_220	15870192	A chromatin immunoprecipitation procedure also has been used to identify DNA binding sites; 203  Drosophila DNA fragments that bind the Engrailed protein were localized in intergenic (53%) or intronic (47%) regions ( ).	bind
41108	3	9431	5	13	NULL	NULL	NULL	statement 1	GP		is localized in									intronic regions	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_20_7097_s_220	15870192	A chromatin immunoprecipitation procedure also has been used to identify DNA binding sites; 203  Drosophila DNA fragments that bind the Engrailed protein were localized in intergenic (53%) or intronic (47%) regions ( ).	bind
41109	4	9431	5	13	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_20_7097_s_220	15870192	A chromatin immunoprecipitation procedure also has been used to identify DNA binding sites; 203  Drosophila DNA fragments that bind the Engrailed protein were localized in intergenic (53%) or intronic (47%) regions ( ).	bind
39767	1	9431	7	NULL	NULL	0	NULL	DNA fragments 	NULL	Drosophila	bind	NULL				Engrailed protein	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_20_7097_s_220	15870192	A chromatin immunoprecipitation procedure also has been used to identify DNA binding sites; 203  Drosophila DNA fragments that bind the Engrailed protein were localized in intergenic (53%) or intronic (47%) regions ( ).	bind
39768	2	9431	7	10	NULL	0	NULL	DNA fragments 		Drosophila	is localized in									intergenic region	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_20_7097_s_220	15870192	A chromatin immunoprecipitation procedure also has been used to identify DNA binding sites; 203  Drosophila DNA fragments that bind the Engrailed protein were localized in intergenic (53%) or intronic (47%) regions ( ).	bind
39769	3	9431	7	10	NULL	0	NULL	DNA fragments 		Drosophila	is localized in									intronic region	NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_20_7097_s_220	15870192	A chromatin immunoprecipitation procedure also has been used to identify DNA binding sites; 203  Drosophila DNA fragments that bind the Engrailed protein were localized in intergenic (53%) or intronic (47%) regions ( ).	bind
56715	4	9431	7	10	NULL	0	NULL	statement 2			is an alternative to					statement 3					NULL		0	NULL	NULL	NULL	gw70_pnas_102_20_7097_s_220	15870192	A chromatin immunoprecipitation procedure also has been used to identify DNA binding sites; 203  Drosophila DNA fragments that bind the Engrailed protein were localized in intergenic (53%) or intronic (47%) regions ( ).	bind
41110	1	9432	5	13	NULL	NULL	NULL	Rox1p	GP		bind					PIS1	NucleicAcid			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_40_38646_s_103	12890676	A circular permutation assay was used to determine whether DNA bending occurred when  Rox1p binds the  PIS1 promoter.	bind
39770	1	9432	7	NULL	NULL	0	NULL	Rox1p	NULL		binds	NULL				 PIS1	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_40_38646_s_103	12890676	A circular permutation assay was used to determine whether DNA bending occurred when  Rox1p binds the  PIS1 promoter.	bind
41111	1	9433	5	13	NULL	NULL	NULL	circulating IgG	GP		bind					beta-adrenoceptor	GP	myocardium			NULL	Chagas disease	NULL	NULL	NULL	NULL	gw60_infectimmun_68_9_5114_s_197	10948133	A circulating IgG in Chagas disease which binds to beta-adrenoceptor of myocardium and modulates their activity.	bind
41112	2	9433	5	13	NULL	NULL	NULL	statement 1	Process		modulates					beta-adrenoceptor	GP	activity of			NULL	Chagas disease	NULL	NULL	NULL	NULL	gw60_infectimmun_68_9_5114_s_197	10948133	A circulating IgG in Chagas disease which binds to beta-adrenoceptor of myocardium and modulates their activity.	bind
39771	1	9433	7	10	NULL	0	NULL	circulating IgG			binds to					beta-adrenoceptor		myocardium			NULL	Chagas disease	NULL	NULL	NULL	NULL	gw60_infectimmun_68_9_5114_s_197	10948133	A circulating IgG in Chagas disease which binds to beta-adrenoceptor of myocardium and modulates their activity.	bind
39772	2	9433	7	10	NULL	0	NULL	statement 1			modulates					beta-adrenoceptor		activity of			NULL	Chagas disease	NULL	NULL	NULL	NULL	gw60_infectimmun_68_9_5114_s_197	10948133	A circulating IgG in Chagas disease which binds to beta-adrenoceptor of myocardium and modulates their activity.	bind
41113	1	9436	5	13	NULL	NULL	NULL	caveolins	GP		is a type of					cellular proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_12_7791_s_16	16299268	A class of cellular proteins named caveolins bind cholesterol at a 1:1 ratio and are involved in transport of de novo-synthesized cholesterol from the ER to the plasma membrane.	bind
41114	2	9436	5	13	NULL	NULL	NULL	caveolins	GP		bind					cholesterol	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_12_7791_s_16	16299268	A class of cellular proteins named caveolins bind cholesterol at a 1:1 ratio and are involved in transport of de novo-synthesized cholesterol from the ER to the plasma membrane.	bind
41115	3	9436	5	13	NULL	NULL	NULL	cholesterol	Chemical	de novo-synthesized	is transported to					plasma membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_12_7791_s_16	16299268	A class of cellular proteins named caveolins bind cholesterol at a 1:1 ratio and are involved in transport of de novo-synthesized cholesterol from the ER to the plasma membrane.	bind
41116	4	9436	5	13	NULL	NULL	NULL	cholesterol	Chemical	de novo-synthesized	is transported from					ER	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_12_7791_s_16	16299268	A class of cellular proteins named caveolins bind cholesterol at a 1:1 ratio and are involved in transport of de novo-synthesized cholesterol from the ER to the plasma membrane.	bind
41117	5	9436	5	13	NULL	NULL	NULL	statement 3	Process		occurs after					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_12_7791_s_16	16299268	A class of cellular proteins named caveolins bind cholesterol at a 1:1 ratio and are involved in transport of de novo-synthesized cholesterol from the ER to the plasma membrane.	bind
56716	6	9436	5	13	NULL	NULL	NULL	caveolins	GP		is involved in					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_12_7791_s_16	16299268	A class of cellular proteins named caveolins bind cholesterol at a 1:1 ratio and are involved in transport of de novo-synthesized cholesterol from the ER to the plasma membrane.	bind
39889	1	9436	7	NULL	NULL	0	NULL	caveolins 	NULL		bind	NULL				cholesterol	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_73_12_7791_s_16	16299268	A class of cellular proteins named caveolins bind cholesterol at a 1:1 ratio and are involved in transport of de novo-synthesized cholesterol from the ER to the plasma membrane.	bind
39890	2	9436	7	10	NULL	0	NULL	cholesterol 	NULL	de novo-synthesized	move from	NULL				ER	NULL				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_12_7791_s_16	16299268	A class of cellular proteins named caveolins bind cholesterol at a 1:1 ratio and are involved in transport of de novo-synthesized cholesterol from the ER to the plasma membrane.	bind
39891	3	9436	7	10	NULL	0	NULL	cholesterol 	NULL	de novo-synthesized 	move to	NULL				plasma membrane	NULL				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_12_7791_s_16	16299268	A class of cellular proteins named caveolins bind cholesterol at a 1:1 ratio and are involved in transport of de novo-synthesized cholesterol from the ER to the plasma membrane.	bind
39892	4	9436	7	NULL	NULL	0	NULL	statement 3	NULL		occurs after	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_73_12_7791_s_16	16299268	A class of cellular proteins named caveolins bind cholesterol at a 1:1 ratio and are involved in transport of de novo-synthesized cholesterol from the ER to the plasma membrane.	bind
39893	5	9436	7	NULL	NULL	0	NULL	caveolins	NULL		is involved in	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_73_12_7791_s_16	16299268	A class of cellular proteins named caveolins bind cholesterol at a 1:1 ratio and are involved in transport of de novo-synthesized cholesterol from the ER to the plasma membrane.	bind
39894	6	9436	7	NULL	NULL	0	NULL	caveolins	NULL		is a type of	NULL				cellular proteins	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_73_12_7791_s_16	16299268	A class of cellular proteins named caveolins bind cholesterol at a 1:1 ratio and are involved in transport of de novo-synthesized cholesterol from the ER to the plasma membrane.	bind
41118	1	9437	5	13	NULL	NULL	NULL	GDP dissociation inhibitors	GP		is critical for					Rab proteins	GP	role of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_34_20470_s_16	8702787	A class of molecules which appear to be critical for the role of Rab proteins are GDP dissociation inhibitors, which bind Rabs that are prenylated (doubly geranylgeranylated near the C terminus) in a specific manner and deliver them to their respective membranes, as well as retrieving them from these locations ( 11).	bind
41119	2	9437	5	13	NULL	NULL	NULL	GDP dissociation inhibitors	GP		bind					Rabs	GP	prenylated			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_34_20470_s_16	8702787	A class of molecules which appear to be critical for the role of Rab proteins are GDP dissociation inhibitors, which bind Rabs that are prenylated (doubly geranylgeranylated near the C terminus) in a specific manner and deliver them to their respective membranes, as well as retrieving them from these locations ( 11).	bind
41121	3	9437	5	13	NULL	NULL	NULL	Rabs	GP	prenylated	is delivered to					membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_34_20470_s_16	8702787	A class of molecules which appear to be critical for the role of Rab proteins are GDP dissociation inhibitors, which bind Rabs that are prenylated (doubly geranylgeranylated near the C terminus) in a specific manner and deliver them to their respective membranes, as well as retrieving them from these locations ( 11).	bind
41122	4	9437	5	13	NULL	NULL	NULL	statement 2	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_34_20470_s_16	8702787	A class of molecules which appear to be critical for the role of Rab proteins are GDP dissociation inhibitors, which bind Rabs that are prenylated (doubly geranylgeranylated near the C terminus) in a specific manner and deliver them to their respective membranes, as well as retrieving them from these locations ( 11).	bind
41124	5	9437	5	13	NULL	NULL	NULL	Rabs	GP	prenylated	is retrieved from					membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_34_20470_s_16	8702787	A class of molecules which appear to be critical for the role of Rab proteins are GDP dissociation inhibitors, which bind Rabs that are prenylated (doubly geranylgeranylated near the C terminus) in a specific manner and deliver them to their respective membranes, as well as retrieving them from these locations ( 11).	bind
41125	6	9437	5	13	NULL	NULL	NULL	statement 2	Process		leads to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_34_20470_s_16	8702787	A class of molecules which appear to be critical for the role of Rab proteins are GDP dissociation inhibitors, which bind Rabs that are prenylated (doubly geranylgeranylated near the C terminus) in a specific manner and deliver them to their respective membranes, as well as retrieving them from these locations ( 11).	bind
39896	2	9437	7	NULL	NULL	0	NULL	geranylgeranylation	NULL		is a type of	NULL	specifically			prenylation	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_34_20470_s_16	8702787	A class of molecules which appear to be critical for the role of Rab proteins are GDP dissociation inhibitors, which bind Rabs that are prenylated (doubly geranylgeranylated near the C terminus) in a specific manner and deliver them to their respective membranes, as well as retrieving them from these locations ( 11).	bind
39897	3	9437	7	NULL	NULL	0	NULL	Rab	NULL		move to	NULL				membranes	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_34_20470_s_16	8702787	A class of molecules which appear to be critical for the role of Rab proteins are GDP dissociation inhibitors, which bind Rabs that are prenylated (doubly geranylgeranylated near the C terminus) in a specific manner and deliver them to their respective membranes, as well as retrieving them from these locations ( 11).	bind
39898	4	9437	7	NULL	NULL	0	NULL	statement 1	NULL		facilitate	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_34_20470_s_16	8702787	A class of molecules which appear to be critical for the role of Rab proteins are GDP dissociation inhibitors, which bind Rabs that are prenylated (doubly geranylgeranylated near the C terminus) in a specific manner and deliver them to their respective membranes, as well as retrieving them from these locations ( 11).	bind
39900	1	9437	7	NULL	NULL	0	NULL	GDP dissociation inhibitors	NULL		bind	NULL				Rab proteins 	NULL	prenylated	C terminus		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_34_20470_s_16	8702787	A class of molecules which appear to be critical for the role of Rab proteins are GDP dissociation inhibitors, which bind Rabs that are prenylated (doubly geranylgeranylated near the C terminus) in a specific manner and deliver them to their respective membranes, as well as retrieving them from these locations ( 11).	bind
39902	5	9437	7	NULL	NULL	0	NULL	Rab	NULL		retreive from	NULL				membranes	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_34_20470_s_16	8702787	A class of molecules which appear to be critical for the role of Rab proteins are GDP dissociation inhibitors, which bind Rabs that are prenylated (doubly geranylgeranylated near the C terminus) in a specific manner and deliver them to their respective membranes, as well as retrieving them from these locations ( 11).	bind
39903	6	9437	7	10	NULL	0	NULL	statement 2	NULL		facilitate	NULL				statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_34_20470_s_16	8702787	A class of molecules which appear to be critical for the role of Rab proteins are GDP dissociation inhibitors, which bind Rabs that are prenylated (doubly geranylgeranylated near the C terminus) in a specific manner and deliver them to their respective membranes, as well as retrieving them from these locations ( 11).	bind
41126	1	9438	5	13	NULL	NULL	NULL	Lip-1	GP		bind					Lyn	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_11_7887_s_90	10713104	A clear association was seen between Lip-1 or Lip-2 and Lyn, with no appreciable binding of Lyn to GST alone (Fig.  1,  B and  C).	bind
41127	2	9438	5	13	NULL	NULL	NULL	Lip-2	GP		bind					Lyn	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_11_7887_s_90	10713104	A clear association was seen between Lip-1 or Lip-2 and Lyn, with no appreciable binding of Lyn to GST alone (Fig.  1,  B and  C).	bind
41128	3	9438	5	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_11_7887_s_90	10713104	A clear association was seen between Lip-1 or Lip-2 and Lyn, with no appreciable binding of Lyn to GST alone (Fig.  1,  B and  C).	bind
39914	1	9438	7	NULL	NULL	0	NULL	Lip-1	NULL		bind	NULL				Lyn	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_11_7887_s_90	10713104	A clear association was seen between Lip-1 or Lip-2 and Lyn, with no appreciable binding of Lyn to GST alone (Fig.  1,  B and  C).	bind
39917	2	9438	7	NULL	NULL	0	NULL	Lip-2	NULL		bind	NULL				Lyn	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_11_7887_s_90	10713104	A clear association was seen between Lip-1 or Lip-2 and Lyn, with no appreciable binding of Lyn to GST alone (Fig.  1,  B and  C).	bind
39918	3	9438	7	10	NULL	0	NULL	statement 1			is an alternative to					statement 2    					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_11_7887_s_90	10713104	A clear association was seen between Lip-1 or Lip-2 and Lyn, with no appreciable binding of Lyn to GST alone (Fig.  1,  B and  C).	bind
41130	1	9439	5	13	NULL	NULL	NULL	RACK1	GP		undergoes					phosphorylation	Process		tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_23_20346_s_320	11279199	A clear correlation exists between enhanced tyrosine phosphorylation of RACK1 and enhanced binding of RACK1 to Src (Figs.  3,  4, and  6).	bind
41131	2	9439	5	13	NULL	NULL	NULL	RACK1	GP		bind					Src	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_23_20346_s_320	11279199	A clear correlation exists between enhanced tyrosine phosphorylation of RACK1 and enhanced binding of RACK1 to Src (Figs.  3,  4, and  6).	bind
41132	3	9439	5	13	NULL	NULL	NULL	statement 1	Process	enhanced	correlates with					statement 2	Process	enhanced			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_23_20346_s_320	11279199	A clear correlation exists between enhanced tyrosine phosphorylation of RACK1 and enhanced binding of RACK1 to Src (Figs.  3,  4, and  6).	bind
39922	1	9439	7	NULL	NULL	0	NULL	RACK1	NULL		bind	NULL				Src	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_23_20346_s_320	11279199	A clear correlation exists between enhanced tyrosine phosphorylation of RACK1 and enhanced binding of RACK1 to Src (Figs.  3,  4, and  6).	bind
39923	2	9439	7	10	NULL	0	NULL	RACK1			undergoes							phosphorylation of 	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_23_20346_s_320	11279199	A clear correlation exists between enhanced tyrosine phosphorylation of RACK1 and enhanced binding of RACK1 to Src (Figs.  3,  4, and  6).	bind
56720	3	9439	7	10	NULL	0	NULL	statement 1		enhanced	correlates with					statement 2		enhanced			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_23_20346_s_320	11279199	A clear correlation exists between enhanced tyrosine phosphorylation of RACK1 and enhanced binding of RACK1 to Src (Figs.  3,  4, and  6).	bind
41133	1	9441	5	13	NULL	NULL	NULL	CSN	GP		cooperates with					Ub - 26S proteasome system	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_7_1630_s_30	11285227	A clear example of CSN and Ub - 26S proteasome system cooperation is the transcription factor c-Jun, which also binds to CSN5/Jab1 ( Claret  et al., 1996).	bind
41134	2	9441	5	13	NULL	NULL	NULL	c-Jun	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_7_1630_s_30	11285227	A clear example of CSN and Ub - 26S proteasome system cooperation is the transcription factor c-Jun, which also binds to CSN5/Jab1 ( Claret  et al., 1996).	bind
41135	3	9441	5	13	NULL	NULL	NULL	c-Jun	GP		bind					CSN5/Jab1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_7_1630_s_30	11285227	A clear example of CSN and Ub - 26S proteasome system cooperation is the transcription factor c-Jun, which also binds to CSN5/Jab1 ( Claret  et al., 1996).	bind
41136	4	9441	5	13	NULL	NULL	NULL	c-Jun	GP		is an example of					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_7_1630_s_30	11285227	A clear example of CSN and Ub - 26S proteasome system cooperation is the transcription factor c-Jun, which also binds to CSN5/Jab1 ( Claret  et al., 1996).	bind
39924	1	9441	7	NULL	NULL	0	NULL	c-Jun	NULL		binds to	NULL				CSN5/Jab1	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_20_7_1630_s_30	11285227	A clear example of CSN and Ub - 26S proteasome system cooperation is the transcription factor c-Jun, which also binds to CSN5/Jab1 ( Claret  et al., 1996).	bind
39925	2	9441	7	NULL	NULL	0	NULL	c-Jun	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_20_7_1630_s_30	11285227	A clear example of CSN and Ub - 26S proteasome system cooperation is the transcription factor c-Jun, which also binds to CSN5/Jab1 ( Claret  et al., 1996).	bind
41264	1	9442	5	13	NULL	NULL	NULL	enzyme	GP		is directed to					site of action	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_26_23874_s_307	12684515	A clear function of the cell wall  binding domain of a peptidoglycan hydrolase is to direct the enzyme to its  site of action, to the poles of the cell in the case of AcmA.	bind
41265	2	9442	5	13	NULL	NULL	NULL	statement 1	GP		function of		clear			peptidoglycan hydrolase	GP		cell wall binding domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_26_23874_s_307	12684515	A clear function of the cell wall  binding domain of a peptidoglycan hydrolase is to direct the enzyme to its  site of action, to the poles of the cell in the case of AcmA.	bind
41266	3	9442	5	13	NULL	NULL	NULL	enzyme	GP		is directed to					cell	Cell	poles of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_26_23874_s_307	12684515	A clear function of the cell wall  binding domain of a peptidoglycan hydrolase is to direct the enzyme to its  site of action, to the poles of the cell in the case of AcmA.	bind
41267	4	9442	5	13	NULL	NULL	NULL	statement 3	Process		function of		clear			AcmA	GP		cell wall binding domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_26_23874_s_307	12684515	A clear function of the cell wall  binding domain of a peptidoglycan hydrolase is to direct the enzyme to its  site of action, to the poles of the cell in the case of AcmA.	bind
39926	1	9442	7	NULL	NULL	0	NULL	enzyme	NULL		move to	NULL				site of action	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_26_23874_s_307	12684515	A clear function of the cell wall  binding domain of a peptidoglycan hydrolase is to direct the enzyme to its  site of action, to the poles of the cell in the case of AcmA.	bind
39927	2	9442	7	NULL	NULL	0	NULL	peptidoglycan hydrolase	NULL		direct	NULL		cell wall binding domain 		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_26_23874_s_307	12684515	A clear function of the cell wall  binding domain of a peptidoglycan hydrolase is to direct the enzyme to its  site of action, to the poles of the cell in the case of AcmA.	bind
39928	3	9442	7	NULL	NULL	0	NULL	AcmA	NULL		move to	NULL				poles of the cell	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_26_23874_s_307	12684515	A clear function of the cell wall  binding domain of a peptidoglycan hydrolase is to direct the enzyme to its  site of action, to the poles of the cell in the case of AcmA.	bind
39929	4	9442	7	NULL	NULL	0	NULL	peptidoglycan hydrolase	NULL		direct	NULL		cell wall binding domain 		statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_26_23874_s_307	12684515	A clear function of the cell wall  binding domain of a peptidoglycan hydrolase is to direct the enzyme to its  site of action, to the poles of the cell in the case of AcmA.	bind
41137	1	9443	5	13	NULL	NULL	NULL	TG	GP		bind		tightly			GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_14_7744_s_111	10869438	A clear rationale for the tight binding of GTP by TG would be to keep the crosslinking activity of the enzyme in check as long as the red cell is to remain in the circulation.	bind
39930	1	9443	7	NULL	NULL	0	NULL	TG	NULL		bind	NULL	tightly			GTP	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_14_7744_s_111	10869438	A clear rationale for the tight binding of GTP by TG would be to keep the crosslinking activity of the enzyme in check as long as the red cell is to remain in the circulation.	bind
41138	1	9445	5	13	NULL	NULL	NULL	MAGE-A4 	GP	cleaved form of	bind					Miz-1	GP				NULL	human cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_15_15505_s_1	14739298	A cleaved form of MAGE-A4 binds to Miz-1 and induces apoptosis in human cells.	bind
41139	2	9445	5	13	NULL	NULL	NULL	statement 1	Process		induce					apoptosis	Process				NULL	human cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_15_15505_s_1	14739298	A cleaved form of MAGE-A4 binds to Miz-1 and induces apoptosis in human cells.	bind
39947	1	9445	7	10	NULL	0	NULL	MAGE-A4		cleaved form of	binds to					Miz-1					NULL	human cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_15_15505_s_1	14739298	A cleaved form of MAGE-A4 binds to Miz-1 and induces apoptosis in human cells.	bind
39948	2	9445	7	NULL	NULL	0	NULL	statement 1	NULL		induce	NULL				apoptosis	NULL				NULL	human cells	0	NULL	NULL	NULL	gw70_jbiolchem_279_15_15505_s_1	14739298	A cleaved form of MAGE-A4 binds to Miz-1 and induces apoptosis in human cells.	bind
41268	1	9447	5	13	NULL	NULL	NULL	cleft	GP		extends from					protomer	GP	center of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_47_48487_s_39	15337754	A cleft extends from the center of the protomer to the central pore of the pentamer, and several residues along the boundaries of this cleft have been shown to be critical for the binding of CRP to C1q, including Asp-112 and Tyr-175 ( ,  ).	bind
41269	2	9447	5	13	NULL	NULL	NULL	cleft	GP		extends to					pentamer	GP	central pore of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_47_48487_s_39	15337754	A cleft extends from the center of the protomer to the central pore of the pentamer, and several residues along the boundaries of this cleft have been shown to be critical for the binding of CRP to C1q, including Asp-112 and Tyr-175 ( ,  ).	bind
41270	3	9447	5	13	NULL	NULL	NULL	CRP	GP		bind					C1q	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_47_48487_s_39	15337754	A cleft extends from the center of the protomer to the central pore of the pentamer, and several residues along the boundaries of this cleft have been shown to be critical for the binding of CRP to C1q, including Asp-112 and Tyr-175 ( ,  ).	bind
41271	4	9447	5	13	NULL	NULL	NULL				is critical for			Asp-112		statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_47_48487_s_39	15337754	A cleft extends from the center of the protomer to the central pore of the pentamer, and several residues along the boundaries of this cleft have been shown to be critical for the binding of CRP to C1q, including Asp-112 and Tyr-175 ( ,  ).	bind
41272	5	9447	5	13	NULL	NULL	NULL				is critical for			Tyr-175		statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_47_48487_s_39	15337754	A cleft extends from the center of the protomer to the central pore of the pentamer, and several residues along the boundaries of this cleft have been shown to be critical for the binding of CRP to C1q, including Asp-112 and Tyr-175 ( ,  ).	bind
41273	6	9447	5	13	NULL	NULL	NULL	statement 5	Process		occurs after					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_47_48487_s_39	15337754	A cleft extends from the center of the protomer to the central pore of the pentamer, and several residues along the boundaries of this cleft have been shown to be critical for the binding of CRP to C1q, including Asp-112 and Tyr-175 ( ,  ).	bind
39949	1	9447	7	NULL	NULL	0	NULL	CRP	NULL		bind	NULL				C1q	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_47_48487_s_39	15337754	A cleft extends from the center of the protomer to the central pore of the pentamer, and several residues along the boundaries of this cleft have been shown to be critical for the binding of CRP to C1q, including Asp-112 and Tyr-175 ( ,  ).	bind
39950	2	9447	7	NULL	NULL	0	NULL		NULL		is critical for	NULL		Asp-112		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_47_48487_s_39	15337754	A cleft extends from the center of the protomer to the central pore of the pentamer, and several residues along the boundaries of this cleft have been shown to be critical for the binding of CRP to C1q, including Asp-112 and Tyr-175 ( ,  ).	bind
39951	3	9447	7	NULL	NULL	0	NULL		NULL		is critical for	NULL		 Tyr-175		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_47_48487_s_39	15337754	A cleft extends from the center of the protomer to the central pore of the pentamer, and several residues along the boundaries of this cleft have been shown to be critical for the binding of CRP to C1q, including Asp-112 and Tyr-175 ( ,  ).	bind
39952	4	9447	7	NULL	NULL	0	NULL	cleft	NULL		extend from	NULL				protomer	NULL	center of the			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_47_48487_s_39	15337754	A cleft extends from the center of the protomer to the central pore of the pentamer, and several residues along the boundaries of this cleft have been shown to be critical for the binding of CRP to C1q, including Asp-112 and Tyr-175 ( ,  ).	bind
39953	5	9447	7	NULL	NULL	0	NULL	cleft 	NULL		extend to	NULL				pentamer	NULL	central pore of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_47_48487_s_39	15337754	A cleft extends from the center of the protomer to the central pore of the pentamer, and several residues along the boundaries of this cleft have been shown to be critical for the binding of CRP to C1q, including Asp-112 and Tyr-175 ( ,  ).	bind
39961	6	9447	7	NULL	NULL	0	NULL	statement 5	NULL		occurs after	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_47_48487_s_39	15337754	A cleft extends from the center of the protomer to the central pore of the pentamer, and several residues along the boundaries of this cleft have been shown to be critical for the binding of CRP to C1q, including Asp-112 and Tyr-175 ( ,  ).	bind
41160	1	9448	5	13	NULL	NULL	NULL	Vi polysaccharide	Chemical	conjugate of	bind					exotoxin A	Chemical	nontoxic;; recombinant;; Pseudomonas aeruginosa			NULL	Vietnamese children	NULL	NULL	NULL	NULL	gw70_clinmicrobiolrev_14_4_872_s_545	11585789	A clinical trial of a conjugate of the Vi polysaccharide bound to nontoxic recombinant  Pseudomonas aeruginosa exotoxin A in Vietnamese children aged 2 to 5 years found the vaccine to be safe and immunogenic ( ).	bind
39962	1	9448	7	10	NULL	0	NULL	Vi polysaccharide		conjugate of	bind					exotoxin A		nontoxic;; recombinant;; Pseudomonas aeruginosa 			NULL	vietnamese children	NULL	NULL	NULL	NULL	gw70_clinmicrobiolrev_14_4_872_s_545	11585789	A clinical trial of a conjugate of the Vi polysaccharide bound to nontoxic recombinant  Pseudomonas aeruginosa exotoxin A in Vietnamese children aged 2 to 5 years found the vaccine to be safe and immunogenic ( ).	bind
41162	1	9450	5	13	NULL	NULL	NULL	AFC2	GP		is a type of					Clk/ty (LAMMER-type) kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_51_36428_s_470	10593939	A Clk/ty (LAMMER-type) kinase (AFC2) binds and phosphorylates all four SR proteins.	bind
41163	2	9450	5	13	NULL	NULL	NULL	AFC2	GP		bind					SR proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_51_36428_s_470	10593939	A Clk/ty (LAMMER-type) kinase (AFC2) binds and phosphorylates all four SR proteins.	bind
41164	3	9450	5	13	NULL	NULL	NULL	statement 1	GP		phosphorylate					SR proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_51_36428_s_470	10593939	A Clk/ty (LAMMER-type) kinase (AFC2) binds and phosphorylates all four SR proteins.	bind
39963	1	9450	7	NULL	NULL	0	NULL	AFC2	NULL		bind	NULL				SR proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_51_36428_s_470	10593939	A Clk/ty (LAMMER-type) kinase (AFC2) binds and phosphorylates all four SR proteins.	bind
39964	2	9450	7	NULL	NULL	0	NULL	AFC2	NULL		phosphorylates	NULL				SR proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_51_36428_s_470	10593939	A Clk/ty (LAMMER-type) kinase (AFC2) binds and phosphorylates all four SR proteins.	bind
39965	3	9450	7	NULL	NULL	0	NULL	AFC2	NULL		is	NULL				Clk/ty (LAMMER-type) kinase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_51_36428_s_470	10593939	A Clk/ty (LAMMER-type) kinase (AFC2) binds and phosphorylates all four SR proteins.	bind
41166	1	9451	5	13	NULL	NULL	NULL	mAb 12G5	GP		bind					CXCR4 coreceptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1587_2_258_s_36	12084468	A close correlation has been found, over a concentration range of 0.1-1000 ng/ml, between the AMD3100 concentrations required to inhibit (i) HIV-1 NL4-3 replication, (ii) monoclonal antibody (mAb 12G5) binding to the CXCR4 coreceptor, and (iii) SDF-1-induced signal transduction (Ca2+ flux), suggesting an intimate relationship between these three parameters [ 29 and  30].	bind
41167	2	9451	5	13	NULL	NULL	NULL	SDF-1	GP		induce					Ca2+ flux	Process	signal transduction of			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1587_2_258_s_36	12084468	A close correlation has been found, over a concentration range of 0.1-1000 ng/ml, between the AMD3100 concentrations required to inhibit (i) HIV-1 NL4-3 replication, (ii) monoclonal antibody (mAb 12G5) binding to the CXCR4 coreceptor, and (iii) SDF-1-induced signal transduction (Ca2+ flux), suggesting an intimate relationship between these three parameters [ 29 and  30].	bind
41168	3	9451	5	13	NULL	NULL	NULL	AMD3100	Chemical		inhibit					HIV-1 NL4-3	Organism	replication of			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1587_2_258_s_36	12084468	A close correlation has been found, over a concentration range of 0.1-1000 ng/ml, between the AMD3100 concentrations required to inhibit (i) HIV-1 NL4-3 replication, (ii) monoclonal antibody (mAb 12G5) binding to the CXCR4 coreceptor, and (iii) SDF-1-induced signal transduction (Ca2+ flux), suggesting an intimate relationship between these three parameters [ 29 and  30].	bind
41169	4	9451	5	13	NULL	NULL	NULL	AMD3100	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1587_2_258_s_36	12084468	A close correlation has been found, over a concentration range of 0.1-1000 ng/ml, between the AMD3100 concentrations required to inhibit (i) HIV-1 NL4-3 replication, (ii) monoclonal antibody (mAb 12G5) binding to the CXCR4 coreceptor, and (iii) SDF-1-induced signal transduction (Ca2+ flux), suggesting an intimate relationship between these three parameters [ 29 and  30].	bind
41170	5	9451	5	13	NULL	NULL	NULL	AMD3100	Chemical		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1587_2_258_s_36	12084468	A close correlation has been found, over a concentration range of 0.1-1000 ng/ml, between the AMD3100 concentrations required to inhibit (i) HIV-1 NL4-3 replication, (ii) monoclonal antibody (mAb 12G5) binding to the CXCR4 coreceptor, and (iii) SDF-1-induced signal transduction (Ca2+ flux), suggesting an intimate relationship between these three parameters [ 29 and  30].	bind
39966	1	9451	7	NULL	NULL	0	NULL	mAb 12G5	NULL		bind	NULL				CXCR4 coreceptor	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1587_2_258_s_36	12084468	A close correlation has been found, over a concentration range of 0.1-1000 ng/ml, between the AMD3100 concentrations required to inhibit (i) HIV-1 NL4-3 replication, (ii) monoclonal antibody (mAb 12G5) binding to the CXCR4 coreceptor, and (iii) SDF-1-induced signal transduction (Ca2+ flux), suggesting an intimate relationship between these three parameters [ 29 and  30].	bind
39967	2	9451	7	NULL	NULL	0	NULL	SDF-1	NULL		induce	NULL				Ca2+ flux	NULL	signal transduction of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1587_2_258_s_36	12084468	A close correlation has been found, over a concentration range of 0.1-1000 ng/ml, between the AMD3100 concentrations required to inhibit (i) HIV-1 NL4-3 replication, (ii) monoclonal antibody (mAb 12G5) binding to the CXCR4 coreceptor, and (iii) SDF-1-induced signal transduction (Ca2+ flux), suggesting an intimate relationship between these three parameters [ 29 and  30].	bind
39968	3	9451	7	NULL	NULL	0	NULL	AMD3100	NULL		inhibit	NULL				HIV-1 NL4-3 	NULL	replication of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1587_2_258_s_36	12084468	A close correlation has been found, over a concentration range of 0.1-1000 ng/ml, between the AMD3100 concentrations required to inhibit (i) HIV-1 NL4-3 replication, (ii) monoclonal antibody (mAb 12G5) binding to the CXCR4 coreceptor, and (iii) SDF-1-induced signal transduction (Ca2+ flux), suggesting an intimate relationship between these three parameters [ 29 and  30].	bind
39969	4	9451	7	NULL	NULL	0	NULL	AMD3100	NULL		inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1587_2_258_s_36	12084468	A close correlation has been found, over a concentration range of 0.1-1000 ng/ml, between the AMD3100 concentrations required to inhibit (i) HIV-1 NL4-3 replication, (ii) monoclonal antibody (mAb 12G5) binding to the CXCR4 coreceptor, and (iii) SDF-1-induced signal transduction (Ca2+ flux), suggesting an intimate relationship between these three parameters [ 29 and  30].	bind
39970	5	9451	7	NULL	NULL	0	NULL	AMD3100	NULL		inhibit	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1587_2_258_s_36	12084468	A close correlation has been found, over a concentration range of 0.1-1000 ng/ml, between the AMD3100 concentrations required to inhibit (i) HIV-1 NL4-3 replication, (ii) monoclonal antibody (mAb 12G5) binding to the CXCR4 coreceptor, and (iii) SDF-1-induced signal transduction (Ca2+ flux), suggesting an intimate relationship between these three parameters [ 29 and  30].	bind
41171	1	9453	5	13	NULL	NULL	NULL	Xylanase	GP	A. niger	is located in				XIP-I binding site	family 11 xylanases	GP		conserved "`thumb"` hairpin loop		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_46_44035_s_10	12207016	A close inspection of the three-dimensional structure of  A. niger xylanase suggests that the binding site of XIP-I is located at the conserved "`thumb"` hairpin loop of family 11 xylanases.	bind
39978	1	9453	7	NULL	NULL	0	NULL	xylanase	NULL	 A. niger	is located in the	NULL		XIP- binding site		family 11 xylanases	NULL		conserved "`thumb"` hairpin loop 		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_46_44035_s_10	12207016	A close inspection of the three-dimensional structure of  A. niger xylanase suggests that the binding site of XIP-I is located at the conserved "`thumb"` hairpin loop of family 11 xylanases.	bind
41172	1	9454	5	13	NULL	NULL	NULL	topo I	GP		bind					plasmid DNA	NucleicAcid	relaxed form of			NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_301_3_789_s_59	12565850	A close up on the DNA-enzyme complexes shown in   Figs. 1D-F demonstrates the binding of topo I to a relaxed form of the plasmid DNA.	bind
39979	1	9454	7	NULL	NULL	0	NULL	topo I	NULL		bind	NULL				plasmid DNA	NULL	relaxed form of			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_301_3_789_s_59	12565850	A close up on the DNA-enzyme complexes shown in   Figs. 1D-F demonstrates the binding of topo I to a relaxed form of the plasmid DNA.	bind
41174	1	9457	5	13	NULL	NULL	NULL	Ank1	GP	muscle	bind					obscurin	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0580-0599_mol-biol-evol_23_1_16135777_s_6	16135777	A closely related sequence in a muscle Ank1  product binds the cytoskeletal muscle proteins obscurin and titin.	bind
41175	2	9457	5	13	NULL	NULL	NULL	Ank1	GP	muscle	bind					titin	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0580-0599_mol-biol-evol_23_1_16135777_s_6	16135777	A closely related sequence in a muscle Ank1  product binds the cytoskeletal muscle proteins obscurin and titin.	bind
41176	3	9457	5	13	NULL	NULL	NULL	titin	GP		is a type of					cytoskeletal muscle proteins	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0580-0599_mol-biol-evol_23_1_16135777_s_6	16135777	A closely related sequence in a muscle Ank1  product binds the cytoskeletal muscle proteins obscurin and titin.	bind
41177	4	9457	5	13	NULL	NULL	NULL	obscurin	GP		is a type of					cytoskeletal muscle proteins	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0580-0599_mol-biol-evol_23_1_16135777_s_6	16135777	A closely related sequence in a muscle Ank1  product binds the cytoskeletal muscle proteins obscurin and titin.	bind
39987	1	9457	7	NULL	NULL	0	NULL	Ank1 product	NULL	muscle	bind	NULL				obscurin	NULL				NULL		0	NULL	NULL	NULL	abs-batch0580-0599_mol-biol-evol_23_1_16135777_s_6	16135777	A closely related sequence in a muscle Ank1  product binds the cytoskeletal muscle proteins obscurin and titin.	bind
39988	2	9457	7	NULL	NULL	0	NULL	Ank1 product	NULL	muscle	bind	NULL				titin	NULL				NULL		0	NULL	NULL	NULL	abs-batch0580-0599_mol-biol-evol_23_1_16135777_s_6	16135777	A closely related sequence in a muscle Ank1  product binds the cytoskeletal muscle proteins obscurin and titin.	bind
39989	3	9457	7	NULL	NULL	0	NULL	obscurin	NULL		is a type of	NULL				cytoskeletal muscle proteins	NULL				NULL		0	NULL	NULL	NULL	abs-batch0580-0599_mol-biol-evol_23_1_16135777_s_6	16135777	A closely related sequence in a muscle Ank1  product binds the cytoskeletal muscle proteins obscurin and titin.	bind
39990	4	9457	7	NULL	NULL	0	NULL	titin	NULL		is a type of	NULL				cytoskeletal muscle protein	NULL				NULL		0	NULL	NULL	NULL	abs-batch0580-0599_mol-biol-evol_23_1_16135777_s_6	16135777	A closely related sequence in a muscle Ank1  product binds the cytoskeletal muscle proteins obscurin and titin.	bind
41276	1	9458	5	13	NULL	NULL	NULL	Sos	GP		bind					Grb2	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_10_5533_s_213	10318918	A closer analysis of NS5A class II motif revealed a complete conservation of the Grb2 N-SH3-binding consensus sequence (PXXPXR), which mediates Sos binding to Grb2.	bind
56721	1	9458	5	13	NULL	NULL	NULL	Grb2	GP		mediates			N-SH3-binding consensus sequence (PXXPXR)		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_10_5533_s_213	10318918	A closer analysis of NS5A class II motif revealed a complete conservation of the Grb2 N-SH3-binding consensus sequence (PXXPXR), which mediates Sos binding to Grb2.	bind
39991	1	9458	7	NULL	NULL	0	NULL	Sos binding	NULL		bind	NULL				Grb2	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_96_10_5533_s_213	10318918	A closer analysis of NS5A class II motif revealed a complete conservation of the Grb2 N-SH3-binding consensus sequence (PXXPXR), which mediates Sos binding to Grb2.	bind
39992	2	9458	7	NULL	NULL	0	NULL	 Grb2	NULL		mediates	NULL		conserved N-SH3-binding consensus sequence (PXXPXR)		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_10_5533_s_213	10318918	A closer analysis of NS5A class II motif revealed a complete conservation of the Grb2 N-SH3-binding consensus sequence (PXXPXR), which mediates Sos binding to Grb2.	bind
41278	1	9459	5	13	NULL	NULL	NULL	zyxin	GP	human	comprise of									alpha-actinin binding site	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_19_13410_s_162	10224105	A closer analysis of the sequence comprising the alpha-actinin binding site of human zyxin showed that it consists of a 10 amino acids submotif occurring twice in tandem (Fig.  5 b).	bind
39994	1	9459	7	10	NULL	0	NULL	zyxin  		human	comprise of									alpha-actinin binding site	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_19_13410_s_162	10224105	A closer analysis of the sequence comprising the alpha-actinin binding site of human zyxin showed that it consists of a 10 amino acids submotif occurring twice in tandem (Fig.  5 b).	bind
41279	1	9460	5	13	NULL	NULL	NULL	ATP/ADP	Chemical		bind					D1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_35_32784_s_247	12807884	A closer examination of   Fig. 7 B revealed that  ATP/ADP binding to D1 does confer a slightly increased protection to the p58  N-D1-linker subcomplex.	bind
41280	2	9460	5	13	NULL	NULL	NULL	statement 1	Process		confer					p58 N-D1-linker subcomplex	GP	increased protection to			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_35_32784_s_247	12807884	A closer examination of   Fig. 7 B revealed that  ATP/ADP binding to D1 does confer a slightly increased protection to the p58  N-D1-linker subcomplex.	bind
39995	1	9460	7	NULL	NULL	0	NULL	ATP/ADP	NULL		bind	NULL				D1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_35_32784_s_247	12807884	A closer examination of   Fig. 7 B revealed that  ATP/ADP binding to D1 does confer a slightly increased protection to the p58  N-D1-linker subcomplex.	bind
39996	2	9460	7	NULL	NULL	0	NULL	statement 1	NULL		increase	NULL				p58 N-D1-linker subcomplex	NULL	protection to			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_35_32784_s_247	12807884	A closer examination of   Fig. 7 B revealed that  ATP/ADP binding to D1 does confer a slightly increased protection to the p58  N-D1-linker subcomplex.	bind
41281	1	9462	5	10	NULL	0	NULL				overlaps			Sp1 site						SF-1 binding element	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17987_s_127	10364248	A closer examination of this sequence revealed a potential Sp1 site, which is overlapping the SF-1 binding element to create an "`Sp1"`FF1 motif (see Fig.  5 B,  probe 2).	bind
41282	2	9462	5	13	NULL	NULL	NULL	statement 1	GP		creates									`Sp1`FF1 motif	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17987_s_127	10364248	A closer examination of this sequence revealed a potential Sp1 site, which is overlapping the SF-1 binding element to create an "`Sp1"`FF1 motif (see Fig.  5 B,  probe 2).	bind
40008	1	9462	7	NULL	NULL	0	NULL		NULL		overlaps with	NULL		Sp1 site			NULL			SF-1 binding element	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_25_17987_s_127	10364248	A closer examination of this sequence revealed a potential Sp1 site, which is overlapping the SF-1 binding element to create an "`Sp1"`FF1 motif (see Fig.  5 B,  probe 2).	bind
40009	2	9462	7	10	NULL	0	NULL	statement 1			create					"`Sp1"`FF1 motif					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17987_s_127	10364248	A closer examination of this sequence revealed a potential Sp1 site, which is overlapping the SF-1 binding element to create an "`Sp1"`FF1 motif (see Fig.  5 B,  probe 2).	bind
41283	1	9463	5	13	NULL	NULL	NULL	hs43	GP		bind		low affinity;;may		ATTG motif in promoter	D-Onecut	GP				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_97_1_57_s_225	11025207	A closer inspection of the  hs43 promoter reveals sequences containing the ATTG motif that may favor low affinity binding to D-Onecut.	bind
40010	1	9463	7	NULL	NULL	0	NULL	hs43	NULL		bind	NULL	low affinity		promoter containing ATTG motif 	D-Onecut	NULL				NULL		0	NULL	NULL	NULL	gw60_mechdev_97_1_57_s_225	11025207	A closer inspection of the  hs43 promoter reveals sequences containing the ATTG motif that may favor low affinity binding to D-Onecut.	bind
41769	1	9464	5	13	NULL	NULL	NULL	YfjB	GP		is a type of					NAD kinases	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_24104_s_112	15855156	A closer inspection of the primary structures of the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p), particularly with respect to the residues (Tyr-202, Ser-205, and Asp-189) participating in the binding of the nicotinamide ring of NAD+ in Ppnk-NAD ( Fig. 1 D), indicated that a residue corresponding to Gly-187 in Ppnk apparently differed between the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p).	bind
41770	2	9464	5	13	NULL	NULL	NULL	NadK	GP		is a type of					NAD kinases	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_24104_s_112	15855156	A closer inspection of the primary structures of the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p), particularly with respect to the residues (Tyr-202, Ser-205, and Asp-189) participating in the binding of the nicotinamide ring of NAD+ in Ppnk-NAD ( Fig. 1 D), indicated that a residue corresponding to Gly-187 in Ppnk apparently differed between the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p).	bind
41771	3	9464	5	13	NULL	NULL	NULL	Mfnk	GP		is a type of					NADH kinases	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_24104_s_112	15855156	A closer inspection of the primary structures of the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p), particularly with respect to the residues (Tyr-202, Ser-205, and Asp-189) participating in the binding of the nicotinamide ring of NAD+ in Ppnk-NAD ( Fig. 1 D), indicated that a residue corresponding to Gly-187 in Ppnk apparently differed between the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p).	bind
41772	4	9464	5	13	NULL	NULL	NULL	Ppnk	GP		is a type of					NADH kinases	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_24104_s_112	15855156	A closer inspection of the primary structures of the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p), particularly with respect to the residues (Tyr-202, Ser-205, and Asp-189) participating in the binding of the nicotinamide ring of NAD+ in Ppnk-NAD ( Fig. 1 D), indicated that a residue corresponding to Gly-187 in Ppnk apparently differed between the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p).	bind
41774	6	9464	5	13	NULL	NULL	NULL	Utr1p	GP		is a type of					NADH kinases	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_24104_s_112	15855156	A closer inspection of the primary structures of the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p), particularly with respect to the residues (Tyr-202, Ser-205, and Asp-189) participating in the binding of the nicotinamide ring of NAD+ in Ppnk-NAD ( Fig. 1 D), indicated that a residue corresponding to Gly-187 in Ppnk apparently differed between the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p).	bind
41775	7	9464	5	13	NULL	NULL	NULL	Yef1p	GP		is a type of					NADH kinases	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_24104_s_112	15855156	A closer inspection of the primary structures of the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p), particularly with respect to the residues (Tyr-202, Ser-205, and Asp-189) participating in the binding of the nicotinamide ring of NAD+ in Ppnk-NAD ( Fig. 1 D), indicated that a residue corresponding to Gly-187 in Ppnk apparently differed between the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p).	bind
41776	8	9464	5	13	NULL	NULL	NULL	Pos5p	GP		is a type of					NADH kinases	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_24104_s_112	15855156	A closer inspection of the primary structures of the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p), particularly with respect to the residues (Tyr-202, Ser-205, and Asp-189) participating in the binding of the nicotinamide ring of NAD+ in Ppnk-NAD ( Fig. 1 D), indicated that a residue corresponding to Gly-187 in Ppnk apparently differed between the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p).	bind
41777	11	9464	5	13	NULL	NULL	NULL	Ppnk-NAD	GP		participate in			Tyr-202		statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_24104_s_112	15855156	A closer inspection of the primary structures of the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p), particularly with respect to the residues (Tyr-202, Ser-205, and Asp-189) participating in the binding of the nicotinamide ring of NAD+ in Ppnk-NAD ( Fig. 1 D), indicated that a residue corresponding to Gly-187 in Ppnk apparently differed between the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p).	bind
41778	10	9464	5	13	NULL	NULL	NULL	Ppnk-NAD	GP		participate in			Ser-205		statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_24104_s_112	15855156	A closer inspection of the primary structures of the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p), particularly with respect to the residues (Tyr-202, Ser-205, and Asp-189) participating in the binding of the nicotinamide ring of NAD+ in Ppnk-NAD ( Fig. 1 D), indicated that a residue corresponding to Gly-187 in Ppnk apparently differed between the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p).	bind
41779	5	9464	5	13	NULL	NULL	NULL	Ppnk-NAD	GP		participate in			Asp-189		statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_24104_s_112	15855156	A closer inspection of the primary structures of the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p), particularly with respect to the residues (Tyr-202, Ser-205, and Asp-189) participating in the binding of the nicotinamide ring of NAD+ in Ppnk-NAD ( Fig. 1 D), indicated that a residue corresponding to Gly-187 in Ppnk apparently differed between the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p).	bind
56722	9	9464	5	13	NULL	NULL	NULL	NAD+	Chemical		bind			nicotinamide ring		Ppnk	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_24104_s_112	15855156	A closer inspection of the primary structures of the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p), particularly with respect to the residues (Tyr-202, Ser-205, and Asp-189) participating in the binding of the nicotinamide ring of NAD+ in Ppnk-NAD ( Fig. 1 D), indicated that a residue corresponding to Gly-187 in Ppnk apparently differed between the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p).	bind
40015	1	9464	7	NULL	NULL	0	NULL	NAD+	NULL		bind	NULL		 nicotinamide ring		Ppnk	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_24104_s_112	15855156	A closer inspection of the primary structures of the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p), particularly with respect to the residues (Tyr-202, Ser-205, and Asp-189) participating in the binding of the nicotinamide ring of NAD+ in Ppnk-NAD ( Fig. 1 D), indicated that a residue corresponding to Gly-187 in Ppnk apparently differed between the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p).	bind
40016	2	9464	7	NULL	NULL	0	NULL	Ppnk	NULL		participate in	NULL		Tyr-202		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_24104_s_112	15855156	A closer inspection of the primary structures of the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p), particularly with respect to the residues (Tyr-202, Ser-205, and Asp-189) participating in the binding of the nicotinamide ring of NAD+ in Ppnk-NAD ( Fig. 1 D), indicated that a residue corresponding to Gly-187 in Ppnk apparently differed between the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p).	bind
40017	3	9464	7	NULL	NULL	0	NULL	Ppnk	NULL		participate in	NULL		Ser-205		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_25_24104_s_112	15855156	A closer inspection of the primary structures of the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p), particularly with respect to the residues (Tyr-202, Ser-205, and Asp-189) participating in the binding of the nicotinamide ring of NAD+ in Ppnk-NAD ( Fig. 1 D), indicated that a residue corresponding to Gly-187 in Ppnk apparently differed between the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p).	bind
40018	4	9464	7	NULL	NULL	0	NULL	Ppnk	NULL		participate in	NULL		 Asp-189		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_25_24104_s_112	15855156	A closer inspection of the primary structures of the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p), particularly with respect to the residues (Tyr-202, Ser-205, and Asp-189) participating in the binding of the nicotinamide ring of NAD+ in Ppnk-NAD ( Fig. 1 D), indicated that a residue corresponding to Gly-187 in Ppnk apparently differed between the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p).	bind
40021	5	9464	7	NULL	NULL	0	NULL	Ppnk	NULL		is a type of	NULL				NADH kinases	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_24104_s_112	15855156	A closer inspection of the primary structures of the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p), particularly with respect to the residues (Tyr-202, Ser-205, and Asp-189) participating in the binding of the nicotinamide ring of NAD+ in Ppnk-NAD ( Fig. 1 D), indicated that a residue corresponding to Gly-187 in Ppnk apparently differed between the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p).	bind
48777	6	9464	7	NULL	NULL	0	NULL	YfjB	NULL		is a type of	NULL				NAD kinases	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_25_24104_s_112	15855156	A closer inspection of the primary structures of the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p), particularly with respect to the residues (Tyr-202, Ser-205, and Asp-189) participating in the binding of the nicotinamide ring of NAD+ in Ppnk-NAD ( Fig. 1 D), indicated that a residue corresponding to Gly-187 in Ppnk apparently differed between the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p).	bind
48778	7	9464	7	NULL	NULL	0	NULL	NadK	NULL		is a type of	NULL				NAD kinases	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_25_24104_s_112	15855156	A closer inspection of the primary structures of the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p), particularly with respect to the residues (Tyr-202, Ser-205, and Asp-189) participating in the binding of the nicotinamide ring of NAD+ in Ppnk-NAD ( Fig. 1 D), indicated that a residue corresponding to Gly-187 in Ppnk apparently differed between the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p).	bind
48779	8	9464	7	NULL	NULL	0	NULL	Mfnk	NULL		is a type of	NULL				NADH kinases	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_25_24104_s_112	15855156	A closer inspection of the primary structures of the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p), particularly with respect to the residues (Tyr-202, Ser-205, and Asp-189) participating in the binding of the nicotinamide ring of NAD+ in Ppnk-NAD ( Fig. 1 D), indicated that a residue corresponding to Gly-187 in Ppnk apparently differed between the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p).	bind
48780	9	9464	7	NULL	NULL	0	NULL	Utr1p	NULL		is a type of	NULL				NADH kinases	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_25_24104_s_112	15855156	A closer inspection of the primary structures of the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p), particularly with respect to the residues (Tyr-202, Ser-205, and Asp-189) participating in the binding of the nicotinamide ring of NAD+ in Ppnk-NAD ( Fig. 1 D), indicated that a residue corresponding to Gly-187 in Ppnk apparently differed between the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p).	bind
48781	10	9464	7	NULL	NULL	0	NULL	Yef1p	NULL		is a type of	NULL				NADH kinases	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_25_24104_s_112	15855156	A closer inspection of the primary structures of the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p), particularly with respect to the residues (Tyr-202, Ser-205, and Asp-189) participating in the binding of the nicotinamide ring of NAD+ in Ppnk-NAD ( Fig. 1 D), indicated that a residue corresponding to Gly-187 in Ppnk apparently differed between the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p).	bind
48782	11	9464	7	NULL	NULL	0	NULL	Pos5p	NULL		is a type of	NULL				NADH kinases	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_24104_s_112	15855156	A closer inspection of the primary structures of the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p), particularly with respect to the residues (Tyr-202, Ser-205, and Asp-189) participating in the binding of the nicotinamide ring of NAD+ in Ppnk-NAD ( Fig. 1 D), indicated that a residue corresponding to Gly-187 in Ppnk apparently differed between the NAD kinases (YfjB and NadK) and the NADH kinases (Mfnk, Ppnk, Utr1p, Yef1p, and Pos5p).	bind
41284	1	9465	5	13	NULL	NULL	NULL	Hop protein	GP		bind			TPR1 domain		Hsp70	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_43_40799_s_287	12145316	A clue can be provided by the Hop protein itself, which binds Hsp70 exclusively through its TPR1 domain and Hsp90 exclusively through its TPR2A domain.	bind
41285	2	9465	5	13	NULL	NULL	NULL	Hop protein	GP		bind			TPR2A domain		Hsp90	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_43_40799_s_287	12145316	A clue can be provided by the Hop protein itself, which binds Hsp70 exclusively through its TPR1 domain and Hsp90 exclusively through its TPR2A domain.	bind
40022	1	9465	7	NULL	NULL	0	NULL	Hop protein	NULL		bind	NULL		TPR1 domain		Hsp70	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_43_40799_s_287	12145316	A clue can be provided by the Hop protein itself, which binds Hsp70 exclusively through its TPR1 domain and Hsp90 exclusively through its TPR2A domain.	bind
40023	2	9465	7	NULL	NULL	0	NULL	Hop protein	NULL		bind	NULL		TPR2A domain		Hsp90	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_43_40799_s_287	12145316	A clue can be provided by the Hop protein itself, which binds Hsp70 exclusively through its TPR1 domain and Hsp90 exclusively through its TPR2A domain.	bind
41286	1	9466	5	13	NULL	NULL	NULL	ATP	Chemical		bind					Smc1/Smc3 heads	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_74_0_595_s_455	15952899	A clue is the finding  that hydrolysis of ATP bound to Smc1/Smc3 heads has an essential role in loading  cohesin onto chromosomes or even onto individual chromatids.	bind
41287	2	9466	5	13	NULL	NULL	NULL	cohesin	GP		loaded onto					chromosomes	Chromosome				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_74_0_595_s_455	15952899	A clue is the finding  that hydrolysis of ATP bound to Smc1/Smc3 heads has an essential role in loading  cohesin onto chromosomes or even onto individual chromatids.	bind
41288	3	9466	5	13	NULL	NULL	NULL	cohesin	GP		loaded onto					chromatids	Chromosome	individual			NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_74_0_595_s_455	15952899	A clue is the finding  that hydrolysis of ATP bound to Smc1/Smc3 heads has an essential role in loading  cohesin onto chromosomes or even onto individual chromatids.	bind
41289	4	9466	5	13	NULL	NULL	NULL	statement 1	Process	hydrolysis of	plays a role in		essential			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_74_0_595_s_455	15952899	A clue is the finding  that hydrolysis of ATP bound to Smc1/Smc3 heads has an essential role in loading  cohesin onto chromosomes or even onto individual chromatids.	bind
41290	5	9466	5	13	NULL	NULL	NULL	statement 1	Process	hydrolysis of	plays a role in		essential			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_74_0_595_s_455	15952899	A clue is the finding  that hydrolysis of ATP bound to Smc1/Smc3 heads has an essential role in loading  cohesin onto chromosomes or even onto individual chromatids.	bind
40024	1	9466	7	NULL	NULL	0	NULL	Smc1/Smc3 heads	NULL		bind	NULL				ATP	NULL				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_74_0_595_s_455	15952899	A clue is the finding  that hydrolysis of ATP bound to Smc1/Smc3 heads has an essential role in loading  cohesin onto chromosomes or even onto individual chromatids.	bind
40025	2	9466	7	NULL	NULL	0	NULL	cohesin	NULL		loaded onto	NULL				chromosomes	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_74_0_595_s_455	15952899	A clue is the finding  that hydrolysis of ATP bound to Smc1/Smc3 heads has an essential role in loading  cohesin onto chromosomes or even onto individual chromatids.	bind
40026	3	9466	7	10	NULL	0	NULL	statement 1	NULL	hydrolysis of	plays a role in	NULL	essential			statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_74_0_595_s_455	15952899	A clue is the finding  that hydrolysis of ATP bound to Smc1/Smc3 heads has an essential role in loading  cohesin onto chromosomes or even onto individual chromatids.	bind
40027	4	9466	7	NULL	NULL	0	NULL	cohesin	NULL		loaded onto	NULL				individual chromatids	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_74_0_595_s_455	15952899	A clue is the finding  that hydrolysis of ATP bound to Smc1/Smc3 heads has an essential role in loading  cohesin onto chromosomes or even onto individual chromatids.	bind
40028	5	9466	7	10	NULL	0	NULL	statement 1	NULL	hydrolysis of	plays a role in	NULL	essential			statement 4	NULL				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_74_0_595_s_455	15952899	A clue is the finding  that hydrolysis of ATP bound to Smc1/Smc3 heads has an essential role in loading  cohesin onto chromosomes or even onto individual chromatids.	bind
41291	1	9467	5	13	NULL	NULL	NULL	IGF-IR	GP		bind			Tyr950		IRS-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_18_12423_s_296	10212216	A clue may be given by reports that the interactions of the IGF-IR with IRS-1 and Shc, although both centered at Tyr950, differ in the requirements for the surrounding amino acids ( 50,  63) and that IRS-1 may also bind directly to the tyrosine kinase domain ( 50).	bind
41292	2	9467	5	13	NULL	NULL	NULL	IGF-IR	GP		bind			Tyr950		Shc	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_18_12423_s_296	10212216	A clue may be given by reports that the interactions of the IGF-IR with IRS-1 and Shc, although both centered at Tyr950, differ in the requirements for the surrounding amino acids ( 50,  63) and that IRS-1 may also bind directly to the tyrosine kinase domain ( 50).	bind
41293	3	9467	5	13	NULL	NULL	NULL	IGF-IR	GP		bind		directly;;may	tyrosine kinase domain		IRS-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_18_12423_s_296	10212216	A clue may be given by reports that the interactions of the IGF-IR with IRS-1 and Shc, although both centered at Tyr950, differ in the requirements for the surrounding amino acids ( 50,  63) and that IRS-1 may also bind directly to the tyrosine kinase domain ( 50).	bind
40029	1	9467	7	10	NULL	0	NULL	IGF-IR			interacts with			Tyr950		IRS-1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_18_12423_s_296	10212216	A clue may be given by reports that the interactions of the IGF-IR with IRS-1 and Shc, although both centered at Tyr950, differ in the requirements for the surrounding amino acids ( 50,  63) and that IRS-1 may also bind directly to the tyrosine kinase domain ( 50).	bind
40030	2	9467	7	10	NULL	0	NULL	IGF-IR			bind			Tyr950		Shc					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_18_12423_s_296	10212216	A clue may be given by reports that the interactions of the IGF-IR with IRS-1 and Shc, although both centered at Tyr950, differ in the requirements for the surrounding amino acids ( 50,  63) and that IRS-1 may also bind directly to the tyrosine kinase domain ( 50).	bind
40033	5	9467	7	10	NULL	0	NULL	IGF-IR			bind		directly;; may	tyrosine kinase domain		IRS-1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_18_12423_s_296	10212216	A clue may be given by reports that the interactions of the IGF-IR with IRS-1 and Shc, although both centered at Tyr950, differ in the requirements for the surrounding amino acids ( 50,  63) and that IRS-1 may also bind directly to the tyrosine kinase domain ( 50).	bind
41294	1	9468	5	13	NULL	NULL	NULL	caspase-3	GP		bind					XIAP	GP		BIR2		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_3_645_s_194	15650747	A clue that the conserved IBM interacting groove may be important for executioner  caspase inhibition is seen in the structure of caspase-3 bound to XIAP BIR2.	bind
41295	2	9468	5	13	NULL	NULL	NULL			conserved	may be important for			IBM interacting groove		statement 1	Process	inhibition of			NULL		NULL	NULL	NULL	NULL	gw70_embo_24_3_645_s_194	15650747	A clue that the conserved IBM interacting groove may be important for executioner  caspase inhibition is seen in the structure of caspase-3 bound to XIAP BIR2.	bind
40036	1	9468	7	10	NULL	0	NULL	caspase-3			bind					XIAP 			BIR2		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_3_645_s_194	15650747	A clue that the conserved IBM interacting groove may be important for executioner  caspase inhibition is seen in the structure of caspase-3 bound to XIAP BIR2.	bind
40037	2	9468	7	10	NULL	0	NULL			conserved	important for		may be	IBM interacting groove		statement 1		inhibition of			NULL		NULL	NULL	NULL	NULL	gw70_embo_24_3_645_s_194	15650747	A clue that the conserved IBM interacting groove may be important for executioner  caspase inhibition is seen in the structure of caspase-3 bound to XIAP BIR2.	bind
41297	1	9469	5	13	NULL	NULL	NULL	FC	GP		bind					Arn1p	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_5_952_s_31	15719020	A clue to the identity of the FC receptor comes from kinetic studies of FC binding  to Arn1p.	bind
40038	1	9469	7	NULL	NULL	0	NULL	FC receptor	NULL		bind	NULL				 Arn1p	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_24_5_952_s_31	15719020	A clue to the identity of the FC receptor comes from kinetic studies of FC binding  to Arn1p.	bind
41298	1	9470	5	13	NULL	NULL	NULL	separin	GP		splits					sister chromatids	Chromosome				NULL		NULL	NULL	NULL	NULL	gw60_science_288_5470_1379_s_185	10827941	A clue to the mechanism by which separin splits sister chromatids was the observation that in budding yeast (contrary to most other eukaryotic cells) most Scc1 remains bound to chromosomes until the metaphase-to-anaphase transition ( 48).	bind
41299	2	9470	5	13	NULL	NULL	NULL	Scc1	GP		bind					chromosomes	Chromosome				NULL	budding yeast	NULL	NULL	NULL	NULL	gw60_science_288_5470_1379_s_185	10827941	A clue to the mechanism by which separin splits sister chromatids was the observation that in budding yeast (contrary to most other eukaryotic cells) most Scc1 remains bound to chromosomes until the metaphase-to-anaphase transition ( 48).	bind
41300	3	9470	5	13	NULL	NULL	NULL	statement 2	Process		until					metaphase-to-anaphase transition 	Process				NULL	budding yeast	NULL	NULL	NULL	NULL	gw60_science_288_5470_1379_s_185	10827941	A clue to the mechanism by which separin splits sister chromatids was the observation that in budding yeast (contrary to most other eukaryotic cells) most Scc1 remains bound to chromosomes until the metaphase-to-anaphase transition ( 48).	bind
41301	4	9470	5	13	NULL	NULL	NULL	statement 2	Process		infers					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_288_5470_1379_s_185	10827941	A clue to the mechanism by which separin splits sister chromatids was the observation that in budding yeast (contrary to most other eukaryotic cells) most Scc1 remains bound to chromosomes until the metaphase-to-anaphase transition ( 48).	bind
40039	1	9470	7	NULL	NULL	0	NULL	separin	NULL		splits	NULL				sister chromatids	NULL				NULL	budding yeast	0	NULL	NULL	NULL	gw60_science_288_5470_1379_s_185	10827941	A clue to the mechanism by which separin splits sister chromatids was the observation that in budding yeast (contrary to most other eukaryotic cells) most Scc1 remains bound to chromosomes until the metaphase-to-anaphase transition ( 48).	bind
40040	2	9470	7	NULL	NULL	0	NULL	Scc1	NULL		bind	NULL				chromosomes	NULL				NULL	budding yeast	NULL	NULL	NULL	NULL	gw60_science_288_5470_1379_s_185	10827941	A clue to the mechanism by which separin splits sister chromatids was the observation that in budding yeast (contrary to most other eukaryotic cells) most Scc1 remains bound to chromosomes until the metaphase-to-anaphase transition ( 48).	bind
40041	3	9470	7	NULL	NULL	0	NULL	chromosomes	NULL		transit from	NULL				metaphase	NULL				NULL	budding yeast	NULL	NULL	NULL	NULL	gw60_science_288_5470_1379_s_185	10827941	A clue to the mechanism by which separin splits sister chromatids was the observation that in budding yeast (contrary to most other eukaryotic cells) most Scc1 remains bound to chromosomes until the metaphase-to-anaphase transition ( 48).	bind
40042	4	9470	7	NULL	NULL	0	NULL	chromosomes	NULL		transit to	NULL				anaphase	NULL				NULL	budding yeast	NULL	NULL	NULL	NULL	gw60_science_288_5470_1379_s_185	10827941	A clue to the mechanism by which separin splits sister chromatids was the observation that in budding yeast (contrary to most other eukaryotic cells) most Scc1 remains bound to chromosomes until the metaphase-to-anaphase transition ( 48).	bind
40043	5	9470	7	NULL	NULL	0	NULL	statement 4	NULL		occurs after	NULL				statement 3	NULL				NULL	budding yeast	NULL	NULL	NULL	NULL	gw60_science_288_5470_1379_s_185	10827941	A clue to the mechanism by which separin splits sister chromatids was the observation that in budding yeast (contrary to most other eukaryotic cells) most Scc1 remains bound to chromosomes until the metaphase-to-anaphase transition ( 48).	bind
40044	6	9470	7	NULL	NULL	0	NULL	statement 1	NULL		occur until	NULL				statement 5	NULL				NULL	budding yeast	NULL	NULL	NULL	NULL	gw60_science_288_5470_1379_s_185	10827941	A clue to the mechanism by which separin splits sister chromatids was the observation that in budding yeast (contrary to most other eukaryotic cells) most Scc1 remains bound to chromosomes until the metaphase-to-anaphase transition ( 48).	bind
41302	1	9471	5	13	NULL	NULL	NULL	Raf-1	GP	endogenous	bind					ERK5	GP	endogenous			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_44_31588_s_4	10531364	A clue to the mechanism of action of Raf-1 on ERK5 comes from the observation that endogenous Raf-1 binds to endogenous ERK5, suggesting the involvement of regulatory protein-protein interactions.	bind
41303	2	9471	5	13	NULL	NULL	NULL	statement 1	Process		suggest					regulatory protein-protein interactions	Process	involvement of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_44_31588_s_4	10531364	A clue to the mechanism of action of Raf-1 on ERK5 comes from the observation that endogenous Raf-1 binds to endogenous ERK5, suggesting the involvement of regulatory protein-protein interactions.	bind
40194	1	9471	7	NULL	NULL	0	NULL	Raf-1	NULL	endogenous	binds to	NULL				ERK5	NULL	endogenous			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_44_31588_s_4	10531364	A clue to the mechanism of action of Raf-1 on ERK5 comes from the observation that endogenous Raf-1 binds to endogenous ERK5, suggesting the involvement of regulatory protein-protein interactions.	bind
40195	2	9471	7	NULL	NULL	0	NULL	statement 1	NULL		suggests	NULL				regulatory protein-protein interactions	NULL	involvement of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_44_31588_s_4	10531364	A clue to the mechanism of action of Raf-1 on ERK5 comes from the observation that endogenous Raf-1 binds to endogenous ERK5, suggesting the involvement of regulatory protein-protein interactions.	bind
41304	1	9472	5	13	NULL	NULL	NULL	EDG-1	GP		overexpressed in					HEK293 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_85	10760461	A clue to the potential physiological function of EDG-1 emerged from the discovery that binding of SPP to EDG-1 overexpressed in HEK293 cells induced up-regulation of P- and E-cadherins, resulting in a distinct morphology of tightly compacted cell-cell aggregates with an organized, network-like architecture and well-developed adherens junctions [ 49].	bind
41305	3	9472	5	13	NULL	NULL	NULL	statement 2	Process		induce					P-cadherins	GP	upregulation of			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_85	10760461	A clue to the potential physiological function of EDG-1 emerged from the discovery that binding of SPP to EDG-1 overexpressed in HEK293 cells induced up-regulation of P- and E-cadherins, resulting in a distinct morphology of tightly compacted cell-cell aggregates with an organized, network-like architecture and well-developed adherens junctions [ 49].	bind
41306	4	9472	5	13	NULL	NULL	NULL	statement 2	Process		induce					E-cadherins	GP	upregulation of			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_85	10760461	A clue to the potential physiological function of EDG-1 emerged from the discovery that binding of SPP to EDG-1 overexpressed in HEK293 cells induced up-regulation of P- and E-cadherins, resulting in a distinct morphology of tightly compacted cell-cell aggregates with an organized, network-like architecture and well-developed adherens junctions [ 49].	bind
41307	2	9472	5	13	NULL	NULL	NULL	SPP	Chemical		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_85	10760461	A clue to the potential physiological function of EDG-1 emerged from the discovery that binding of SPP to EDG-1 overexpressed in HEK293 cells induced up-regulation of P- and E-cadherins, resulting in a distinct morphology of tightly compacted cell-cell aggregates with an organized, network-like architecture and well-developed adherens junctions [ 49].	bind
41308	5	9472	5	13	NULL	NULL	NULL	cell-cell aggregates	Process		is compacted					tightly 					NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_85	10760461	A clue to the potential physiological function of EDG-1 emerged from the discovery that binding of SPP to EDG-1 overexpressed in HEK293 cells induced up-regulation of P- and E-cadherins, resulting in a distinct morphology of tightly compacted cell-cell aggregates with an organized, network-like architecture and well-developed adherens junctions [ 49].	bind
41309	6	9472	5	13	NULL	NULL	NULL	statement 5	Process		contains					architecture		organized;;network-like			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_85	10760461	A clue to the potential physiological function of EDG-1 emerged from the discovery that binding of SPP to EDG-1 overexpressed in HEK293 cells induced up-regulation of P- and E-cadherins, resulting in a distinct morphology of tightly compacted cell-cell aggregates with an organized, network-like architecture and well-developed adherens junctions [ 49].	bind
41310	7	9472	5	13	NULL	NULL	NULL	statement 5	Process		contains					adherens junctions	CellComponent	well-developed			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_85	10760461	A clue to the potential physiological function of EDG-1 emerged from the discovery that binding of SPP to EDG-1 overexpressed in HEK293 cells induced up-regulation of P- and E-cadherins, resulting in a distinct morphology of tightly compacted cell-cell aggregates with an organized, network-like architecture and well-developed adherens junctions [ 49].	bind
41311	8	9472	5	13	NULL	NULL	NULL	statement 3	Process		results in					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_85	10760461	A clue to the potential physiological function of EDG-1 emerged from the discovery that binding of SPP to EDG-1 overexpressed in HEK293 cells induced up-regulation of P- and E-cadherins, resulting in a distinct morphology of tightly compacted cell-cell aggregates with an organized, network-like architecture and well-developed adherens junctions [ 49].	bind
41312	9	9472	5	13	NULL	NULL	NULL	statement 3	Process		results in					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_85	10760461	A clue to the potential physiological function of EDG-1 emerged from the discovery that binding of SPP to EDG-1 overexpressed in HEK293 cells induced up-regulation of P- and E-cadherins, resulting in a distinct morphology of tightly compacted cell-cell aggregates with an organized, network-like architecture and well-developed adherens junctions [ 49].	bind
41313	10	9472	5	13	NULL	NULL	NULL	statement 4	Process		results in					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_85	10760461	A clue to the potential physiological function of EDG-1 emerged from the discovery that binding of SPP to EDG-1 overexpressed in HEK293 cells induced up-regulation of P- and E-cadherins, resulting in a distinct morphology of tightly compacted cell-cell aggregates with an organized, network-like architecture and well-developed adherens junctions [ 49].	bind
41314	11	9472	5	13	NULL	NULL	NULL	statement 4	Process		results in					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_85	10760461	A clue to the potential physiological function of EDG-1 emerged from the discovery that binding of SPP to EDG-1 overexpressed in HEK293 cells induced up-regulation of P- and E-cadherins, resulting in a distinct morphology of tightly compacted cell-cell aggregates with an organized, network-like architecture and well-developed adherens junctions [ 49].	bind
40196	1	9472	7	10	NULL	0	NULL	SPP			bind					statement 10					NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_85	10760461	A clue to the potential physiological function of EDG-1 emerged from the discovery that binding of SPP to EDG-1 overexpressed in HEK293 cells induced up-regulation of P- and E-cadherins, resulting in a distinct morphology of tightly compacted cell-cell aggregates with an organized, network-like architecture and well-developed adherens junctions [ 49].	bind
40197	2	9472	7	NULL	NULL	0	NULL	statement 1	NULL		induce	NULL				P-cadherins	NULL	upregulation of			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_85	10760461	A clue to the potential physiological function of EDG-1 emerged from the discovery that binding of SPP to EDG-1 overexpressed in HEK293 cells induced up-regulation of P- and E-cadherins, resulting in a distinct morphology of tightly compacted cell-cell aggregates with an organized, network-like architecture and well-developed adherens junctions [ 49].	bind
40198	3	9472	7	NULL	NULL	0	NULL	statement 1	NULL		induce	NULL				E-cadherins	NULL	upregulation of			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_85	10760461	A clue to the potential physiological function of EDG-1 emerged from the discovery that binding of SPP to EDG-1 overexpressed in HEK293 cells induced up-regulation of P- and E-cadherins, resulting in a distinct morphology of tightly compacted cell-cell aggregates with an organized, network-like architecture and well-developed adherens junctions [ 49].	bind
40199	4	9472	7	NULL	NULL	0	NULL	statement 2	NULL		result in	NULL				cell-cell aggregates	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_85	10760461	A clue to the potential physiological function of EDG-1 emerged from the discovery that binding of SPP to EDG-1 overexpressed in HEK293 cells induced up-regulation of P- and E-cadherins, resulting in a distinct morphology of tightly compacted cell-cell aggregates with an organized, network-like architecture and well-developed adherens junctions [ 49].	bind
40200	5	9472	7	NULL	NULL	0	NULL	statement 3	NULL		result in	NULL				cell-cell aggregates	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_85	10760461	A clue to the potential physiological function of EDG-1 emerged from the discovery that binding of SPP to EDG-1 overexpressed in HEK293 cells induced up-regulation of P- and E-cadherins, resulting in a distinct morphology of tightly compacted cell-cell aggregates with an organized, network-like architecture and well-developed adherens junctions [ 49].	bind
40206	6	9472	7	NULL	NULL	0	NULL	statement 4	NULL		result in	NULL				 organized network-like architecture	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_85	10760461	A clue to the potential physiological function of EDG-1 emerged from the discovery that binding of SPP to EDG-1 overexpressed in HEK293 cells induced up-regulation of P- and E-cadherins, resulting in a distinct morphology of tightly compacted cell-cell aggregates with an organized, network-like architecture and well-developed adherens junctions [ 49].	bind
40208	7	9472	7	10	NULL	0	NULL	statement 5	NULL		result in	NULL				network-like architecture	NULL	organized 			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_85	10760461	A clue to the potential physiological function of EDG-1 emerged from the discovery that binding of SPP to EDG-1 overexpressed in HEK293 cells induced up-regulation of P- and E-cadherins, resulting in a distinct morphology of tightly compacted cell-cell aggregates with an organized, network-like architecture and well-developed adherens junctions [ 49].	bind
40211	8	9472	7	10	NULL	0	NULL	statement 4	NULL		result in	NULL				adherens junctions	NULL	well-developed 			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_85	10760461	A clue to the potential physiological function of EDG-1 emerged from the discovery that binding of SPP to EDG-1 overexpressed in HEK293 cells induced up-regulation of P- and E-cadherins, resulting in a distinct morphology of tightly compacted cell-cell aggregates with an organized, network-like architecture and well-developed adherens junctions [ 49].	bind
40212	9	9472	7	10	NULL	0	NULL	statement 5	NULL		result in	NULL				adherens junctions	NULL	well-developed			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_85	10760461	A clue to the potential physiological function of EDG-1 emerged from the discovery that binding of SPP to EDG-1 overexpressed in HEK293 cells induced up-regulation of P- and E-cadherins, resulting in a distinct morphology of tightly compacted cell-cell aggregates with an organized, network-like architecture and well-developed adherens junctions [ 49].	bind
56723	10	9472	7	10	NULL	0	NULL	EDG-1			overexpressed in					HEK293 cells					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_85	10760461	A clue to the potential physiological function of EDG-1 emerged from the discovery that binding of SPP to EDG-1 overexpressed in HEK293 cells induced up-regulation of P- and E-cadherins, resulting in a distinct morphology of tightly compacted cell-cell aggregates with an organized, network-like architecture and well-developed adherens junctions [ 49].	bind
41315	1	9473	5	13	NULL	NULL	NULL	F-actin	GP		bind					dystrophin	GP		cluster of basic repeats		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_1_153_s_372	10189375	A cluster of basic repeats in  the dystrophin rod domain binds F-actin through an electrostatic interaction.	bind
41317	2	9473	5	13	NULL	NULL	NULL	statement 1	Process		occurs through					electrostatic interaction	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_1_153_s_372	10189375	A cluster of basic repeats in  the dystrophin rod domain binds F-actin through an electrostatic interaction.	bind
40213	1	9473	7	NULL	NULL	0	NULL	dystrophin	NULL		binds	NULL		basic repeats in rod domain		F-actin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_1_153_s_372	10189375	A cluster of basic repeats in  the dystrophin rod domain binds F-actin through an electrostatic interaction.	bind
40214	2	9473	7	NULL	NULL	0	NULL	statement 1	NULL		occurs through	NULL				electrostatic interactions	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_1_153_s_372	10189375	A cluster of basic repeats in  the dystrophin rod domain binds F-actin through an electrostatic interaction.	bind
41318	1	9475	5	13	NULL	NULL	NULL	DnaA protein molecules	GP		bind					DnaA	GP			recognition sites in oriC	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_9796_s_9	15642730	A cluster of multiple DnaA protein molecules binds to DnaA recognition sites in the unique origin ( oriC) (  -  ).	bind
41319	2	9475	5	13	NULL	NULL	NULL	oriC	NucleicAcid		is					unique origin	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_9796_s_9	15642730	A cluster of multiple DnaA protein molecules binds to DnaA recognition sites in the unique origin ( oriC) (  -  ).	bind
56724	2	9475	5	13	NULL	NULL	NULL	oriC	NucleicAcid		is					unique origin	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_9796_s_9	15642730	A cluster of multiple DnaA protein molecules binds to DnaA recognition sites in the unique origin ( oriC) (  -  ).	bind
56725	2	9475	5	13	NULL	NULL	NULL	oriC	NucleicAcid		is					unique origin	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_9796_s_9	15642730	A cluster of multiple DnaA protein molecules binds to DnaA recognition sites in the unique origin ( oriC) (  -  ).	bind
40218	1	9475	7	NULL	NULL	0	NULL	DnaA protein molecules	NULL		bind	NULL				oriC	NULL		DnaA recognition site		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_11_9796_s_9	15642730	A cluster of multiple DnaA protein molecules binds to DnaA recognition sites in the unique origin ( oriC) (  -  ).	bind
41320	1	9476	5	13	NULL	NULL	NULL	p21	GP		bind			cluster of serine and threonine residues in C-terminal domain		PCNA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_15_11529_s_123	10753973	A cluster of serine and threonine residues is present within the C-terminal domain of p21 that binds to PCNA, and a "`motif"` search identified three of these residues as lying within possible consensus phosphorylation sites.	bind
40221	1	9476	7	NULL	NULL	0	NULL	p21	NULL		binds to	NULL		cluster of serine and threonine residues in C-terminal domain		PCNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_15_11529_s_123	10753973	A cluster of serine and threonine residues is present within the C-terminal domain of p21 that binds to PCNA, and a "`motif"` search identified three of these residues as lying within possible consensus phosphorylation sites.	bind
41322	1	9478	5	13	NULL	NULL	NULL	CNS-enriched factor	GP		bind					NF-kappa B	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_oncogene_10_2_7838536_s_1	7838536	A CNS-enriched factor that binds to NF-kappa B and is required for interaction with HIV-1 tat..	bind
41323	2	9478	5	13	NULL	NULL	NULL	statement 1	GP		is required for					HIV-1 tat	GP	interaction with			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_oncogene_10_2_7838536_s_1	7838536	A CNS-enriched factor that binds to NF-kappa B and is required for interaction with HIV-1 tat..	bind
40252	1	9478	7	NULL	NULL	0	NULL	CNS-enriched factor	NULL		binds to	NULL				NF-kappa B	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_oncogene_10_2_7838536_s_1	7838536	A CNS-enriched factor that binds to NF-kappa B and is required for interaction with HIV-1 tat..	bind
40253	2	9478	7	NULL	NULL	0	NULL	statement 1	NULL		is required for	NULL				HIV-1 tat	NULL	interaction of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_oncogene_10_2_7838536_s_1	7838536	A CNS-enriched factor that binds to NF-kappa B and is required for interaction with HIV-1 tat..	bind
41329	1	9479	5	13	NULL	NULL	NULL	heparin	Chemical		bind					basic fibroblast growth factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_13_12598_s_26	14707146	A co-crystal structure is available for heparin bound to the cytokine basic fibroblast growth factor ( ), but the features governing protein-GAG recognition are still relatively uncharacterized.	bind
41330	2	9479	5	13	NULL	NULL	NULL	basic fibroblast growth factor	GP		is a type of					cytokine	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_13_12598_s_26	14707146	A co-crystal structure is available for heparin bound to the cytokine basic fibroblast growth factor ( ), but the features governing protein-GAG recognition are still relatively uncharacterized.	bind
40254	1	9479	7	10	NULL	0	NULL	heparin	NULL		bind	NULL				basic fibroblast growth factor	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_13_12598_s_26	14707146	A co-crystal structure is available for heparin bound to the cytokine basic fibroblast growth factor ( ), but the features governing protein-GAG recognition are still relatively uncharacterized.	bind
46842	2	9479	7	10	NULL	0	NULL	basic fibroblast growth factor	NULL		is a type of 	NULL				cytokine	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12598_s_26	14707146	A co-crystal structure is available for heparin bound to the cytokine basic fibroblast growth factor ( ), but the features governing protein-GAG recognition are still relatively uncharacterized.	bind
41331	1	9480	5	13	NULL	NULL	NULL	peptide aldehyde inhibitor	GP		bind		covalently			Pre3	GP		terminal threonines		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25200_s_275	9312134	A co-crystallized peptide aldehyde inhibitor was found covalently bound to the terminal threonines of Pre3, Pup1, and Pre2.	bind
41332	2	9480	5	13	NULL	NULL	NULL	peptide aldehyde inhibitor	GP		bind		covalently			Pre2	GP		terminal threonines		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25200_s_275	9312134	A co-crystallized peptide aldehyde inhibitor was found covalently bound to the terminal threonines of Pre3, Pup1, and Pre2.	bind
41333	3	9480	5	13	NULL	NULL	NULL	peptide aldehyde inhibitor	GP		bind		covalently			Pup1	GP		terminal threonines		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25200_s_275	9312134	A co-crystallized peptide aldehyde inhibitor was found covalently bound to the terminal threonines of Pre3, Pup1, and Pre2.	bind
40255	1	9480	7	NULL	NULL	0	NULL	peptide aldehyde inhibitor	NULL		bind	NULL	covalently			Pre3	NULL		 terminal threonine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25200_s_275	9312134	A co-crystallized peptide aldehyde inhibitor was found covalently bound to the terminal threonines of Pre3, Pup1, and Pre2.	bind
40256	2	9480	7	NULL	NULL	0	NULL	peptide aldehyde inhibitor	NULL		bind	NULL	covalently			Pup1	NULL		terminal threonine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25200_s_275	9312134	A co-crystallized peptide aldehyde inhibitor was found covalently bound to the terminal threonines of Pre3, Pup1, and Pre2.	bind
40257	3	9480	7	NULL	NULL	0	NULL	peptide aldehyde inhibitor	NULL		bind	NULL	covalently			Pre2	NULL		terminal threonine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_40_25200_s_275	9312134	A co-crystallized peptide aldehyde inhibitor was found covalently bound to the terminal threonines of Pre3, Pup1, and Pre2.	bind
41334	1	9482	5	13	NULL	NULL	NULL	EGL-1	GP		bind		stably			CED-9	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_cell-death-differ_10_12_12894216_s_4	12894216	A coexpression system to  produce CED-9 in complex with proapoptotic EGL-1 enabled us to show that  the binding of EGL-1 to CED-9 is extremely stable, raising the melting  temperature (T(M)) of CED-9 by 25 degrees C, and that the binding surface  of CED-9 extends beyond the BH3-binding region and reaches the BH4 domain.	bind
41335	2	9482	5	13	NULL	NULL	NULL	CED-9	GP	binding surface of	extends beyond								BH3-binding region		NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_cell-death-differ_10_12_12894216_s_4	12894216	A coexpression system to  produce CED-9 in complex with proapoptotic EGL-1 enabled us to show that  the binding of EGL-1 to CED-9 is extremely stable, raising the melting  temperature (T(M)) of CED-9 by 25 degrees C, and that the binding surface  of CED-9 extends beyond the BH3-binding region and reaches the BH4 domain.	bind
41336	3	9482	5	13	NULL	NULL	NULL	CED-9	GP	binding surface of	reaches								BH4 domain		NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_cell-death-differ_10_12_12894216_s_4	12894216	A coexpression system to  produce CED-9 in complex with proapoptotic EGL-1 enabled us to show that  the binding of EGL-1 to CED-9 is extremely stable, raising the melting  temperature (T(M)) of CED-9 by 25 degrees C, and that the binding surface  of CED-9 extends beyond the BH3-binding region and reaches the BH4 domain.	bind
40260	1	9482	7	NULL	NULL	0	NULL	EGL-1	NULL		bind	NULL				CED-9	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_cell-death-differ_10_12_12894216_s_4	12894216	A coexpression system to  produce CED-9 in complex with proapoptotic EGL-1 enabled us to show that  the binding of EGL-1 to CED-9 is extremely stable, raising the melting  temperature (T(M)) of CED-9 by 25 degrees C, and that the binding surface  of CED-9 extends beyond the BH3-binding region and reaches the BH4 domain.	bind
40263	2	9482	7	10	NULL	0	NULL	CED-9		binding surface of	extends beyond								BH3-binding region		NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_cell-death-differ_10_12_12894216_s_4	12894216	A coexpression system to  produce CED-9 in complex with proapoptotic EGL-1 enabled us to show that  the binding of EGL-1 to CED-9 is extremely stable, raising the melting  temperature (T(M)) of CED-9 by 25 degrees C, and that the binding surface  of CED-9 extends beyond the BH3-binding region and reaches the BH4 domain.	bind
40264	3	9482	7	10	NULL	0	NULL	CED-9		binding surface of	reaches								BH4 domain		NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_cell-death-differ_10_12_12894216_s_4	12894216	A coexpression system to  produce CED-9 in complex with proapoptotic EGL-1 enabled us to show that  the binding of EGL-1 to CED-9 is extremely stable, raising the melting  temperature (T(M)) of CED-9 by 25 degrees C, and that the binding surface  of CED-9 extends beyond the BH3-binding region and reaches the BH4 domain.	bind
41337	1	9483	5	13	NULL	NULL	NULL	mod(mdg4)	Chemical		bind					su(Hw)	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_3_271_s_75	11825869	A cofactor, mod(mdg4), binds to su(Hw) and is essential for its enhancer-blocking activity (see below; Gerasimova et al. 1995  ).	bind
41338	2	9483	5	13	NULL	NULL	NULL	mod(mdg4)	Chemical		exhibits					enhancer-blocking activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_3_271_s_75	11825869	A cofactor, mod(mdg4), binds to su(Hw) and is essential for its enhancer-blocking activity (see below; Gerasimova et al. 1995  ).	bind
41339	3	9483	5	13	NULL	NULL	NULL	mod(mdg4)	Chemical		is a type of					cofactor	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_3_271_s_75	11825869	A cofactor, mod(mdg4), binds to su(Hw) and is essential for its enhancer-blocking activity (see below; Gerasimova et al. 1995  ).	bind
46843	4	9483	5	13	NULL	NULL	NULL	statement 1	Process		is essential for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_3_271_s_75	11825869	A cofactor, mod(mdg4), binds to su(Hw) and is essential for its enhancer-blocking activity (see below; Gerasimova et al. 1995  ).	bind
40275	1	9483	7	NULL	NULL	0	NULL	mdg4	NULL		binds to	NULL				su(Hw)	NULL				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_3_271_s_75	11825869	A cofactor, mod(mdg4), binds to su(Hw) and is essential for its enhancer-blocking activity (see below; Gerasimova et al. 1995  ).	bind
40276	2	9483	7	10	NULL	0	NULL	mod(mdg4)	NULL		exhibits	NULL				enhancer-blocking activity	NULL				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_3_271_s_75	11825869	A cofactor, mod(mdg4), binds to su(Hw) and is essential for its enhancer-blocking activity (see below; Gerasimova et al. 1995  ).	bind
40277	3	9483	7	NULL	NULL	0	NULL	mdg4	NULL		is a type of	NULL				cofactor mod	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_16_3_271_s_75	11825869	A cofactor, mod(mdg4), binds to su(Hw) and is essential for its enhancer-blocking activity (see below; Gerasimova et al. 1995  ).	bind
46844	4	9483	7	10	NULL	0	NULL	statement 1	NULL		is essential for	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_16_3_271_s_75	11825869	A cofactor, mod(mdg4), binds to su(Hw) and is essential for its enhancer-blocking activity (see below; Gerasimova et al. 1995  ).	bind
41340	1	9486	5	13	NULL	NULL	NULL	p34	GP		bind					22 S dynein	GP	Paramecium			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_23_20048_s_173	11274140	A cold-labeled p29 fraction was added at increasing concentrations to compete with binding of p34 to  Paramecium 22 S dynein.	bind
40278	1	9486	7	NULL	NULL	0	NULL	 p34	NULL		bind	NULL				22 S dynein	NULL	Paramecium			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_23_20048_s_173	11274140	A cold-labeled p29 fraction was added at increasing concentrations to compete with binding of p34 to  Paramecium 22 S dynein.	bind
40279	2	9486	7	NULL	NULL	0	NULL	p29 fraction	NULL	cold-labeled	bind	NULL				22 S dynein	NULL	Paramecium			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_23_20048_s_173	11274140	A cold-labeled p29 fraction was added at increasing concentrations to compete with binding of p34 to  Paramecium 22 S dynein.	bind
40280	3	9486	7	NULL	NULL	0	NULL	statement 2	NULL		compete with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_23_20048_s_173	11274140	A cold-labeled p29 fraction was added at increasing concentrations to compete with binding of p34 to  Paramecium 22 S dynein.	bind
41341	1	9487	5	13	NULL	NULL	NULL	fibromodulin	GP		is a type of					collagen binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_genomeres_9_5_449_s_341	10330124	A collagen binding 59 kD protein (fibromodulin) is structurally related to the small interstitial proteoglycans PG S1 and PG S2 (decorin).	bind
41342	2	9487	5	13	NULL	NULL	NULL	fibromodulin	GP		is related to					PG S1	GP				NULL		NULL	NULL	NULL	NULL	gw60_genomeres_9_5_449_s_341	10330124	A collagen binding 59 kD protein (fibromodulin) is structurally related to the small interstitial proteoglycans PG S1 and PG S2 (decorin).	bind
41343	3	9487	5	13	NULL	NULL	NULL	fibromodulin	GP		is related to					PG S2	GP				NULL		NULL	NULL	NULL	NULL	gw60_genomeres_9_5_449_s_341	10330124	A collagen binding 59 kD protein (fibromodulin) is structurally related to the small interstitial proteoglycans PG S1 and PG S2 (decorin).	bind
41344	4	9487	5	13	NULL	NULL	NULL	PG S1	GP		is a type of					small interstitial proteoglycans	GP				NULL		NULL	NULL	NULL	NULL	gw60_genomeres_9_5_449_s_341	10330124	A collagen binding 59 kD protein (fibromodulin) is structurally related to the small interstitial proteoglycans PG S1 and PG S2 (decorin).	bind
41345	5	9487	5	13	NULL	NULL	NULL	PG S2	GP		is a type of					small interstitial proteoglycans	GP				NULL		NULL	NULL	NULL	NULL	gw60_genomeres_9_5_449_s_341	10330124	A collagen binding 59 kD protein (fibromodulin) is structurally related to the small interstitial proteoglycans PG S1 and PG S2 (decorin).	bind
41346	6	9487	5	13	NULL	NULL	NULL	PG S2	GP		is					decorin	GP				NULL		NULL	NULL	NULL	NULL	gw60_genomeres_9_5_449_s_341	10330124	A collagen binding 59 kD protein (fibromodulin) is structurally related to the small interstitial proteoglycans PG S1 and PG S2 (decorin).	bind
40281	1	9487	7	NULL	NULL	0	NULL	fibromodulin	NULL		bind	NULL				collagen	NULL				NULL		NULL	NULL	NULL	NULL	gw60_genomeres_9_5_449_s_341	10330124	A collagen binding 59 kD protein (fibromodulin) is structurally related to the small interstitial proteoglycans PG S1 and PG S2 (decorin).	bind
40282	2	9487	7	NULL	NULL	0	NULL	fibromodulin	NULL		is a type of	NULL				59 kD protein	NULL				NULL		0	NULL	NULL	NULL	gw60_genomeres_9_5_449_s_341	10330124	A collagen binding 59 kD protein (fibromodulin) is structurally related to the small interstitial proteoglycans PG S1 and PG S2 (decorin).	bind
40283	3	9487	7	NULL	NULL	0	NULL	fibromodulin	NULL		is related to	NULL				PG S1	NULL				NULL		0	NULL	NULL	NULL	gw60_genomeres_9_5_449_s_341	10330124	A collagen binding 59 kD protein (fibromodulin) is structurally related to the small interstitial proteoglycans PG S1 and PG S2 (decorin).	bind
40284	4	9487	7	NULL	NULL	0	NULL	fibromodulin	NULL		is related to	NULL				PG S2	NULL				NULL		0	NULL	NULL	NULL	gw60_genomeres_9_5_449_s_341	10330124	A collagen binding 59 kD protein (fibromodulin) is structurally related to the small interstitial proteoglycans PG S1 and PG S2 (decorin).	bind
40286	5	9487	7	NULL	NULL	0	NULL	PG S1	NULL		is a type of	NULL				small interstitial proteoglycans	NULL				NULL		0	NULL	NULL	NULL	gw60_genomeres_9_5_449_s_341	10330124	A collagen binding 59 kD protein (fibromodulin) is structurally related to the small interstitial proteoglycans PG S1 and PG S2 (decorin).	bind
40287	6	9487	7	NULL	NULL	0	NULL	PG S2	NULL		is a type of	NULL				small interstitial proteoglycans	NULL				NULL		0	NULL	NULL	NULL	gw60_genomeres_9_5_449_s_341	10330124	A collagen binding 59 kD protein (fibromodulin) is structurally related to the small interstitial proteoglycans PG S1 and PG S2 (decorin).	bind
40288	7	9487	7	NULL	NULL	0	NULL	PG S2	NULL		is 	NULL				decorin	NULL				NULL		0	NULL	NULL	NULL	gw60_genomeres_9_5_449_s_341	10330124	A collagen binding 59 kD protein (fibromodulin) is structurally related to the small interstitial proteoglycans PG S1 and PG S2 (decorin).	bind
41349	1	9489	5	13	NULL	NULL	NULL	ShcB	GP		bind			Tyr499		TrkA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_29_26046_s_210	12006576	A combination mutation of S8 and S9 also significantly reduced the binding of ShcB to TrkA (Fig.  2 B,  top panel,  lane 6), which confirmed that Tyr499 is the binding site of ShcB to TrkA.	bind
41350	2	9489	5	13	NULL	NULL	NULL			mutant	reduce		significantly	S8		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_29_26046_s_210	12006576	A combination mutation of S8 and S9 also significantly reduced the binding of ShcB to TrkA (Fig.  2 B,  top panel,  lane 6), which confirmed that Tyr499 is the binding site of ShcB to TrkA.	bind
41351	3	9489	5	13	NULL	NULL	NULL			mutant	reduce		significantly	S9		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_29_26046_s_210	12006576	A combination mutation of S8 and S9 also significantly reduced the binding of ShcB to TrkA (Fig.  2 B,  top panel,  lane 6), which confirmed that Tyr499 is the binding site of ShcB to TrkA.	bind
40300	1	9489	7	NULL	NULL	0	NULL	ShcB 	NULL		bind	NULL		Tyr499		TrkA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26046_s_210	12006576	A combination mutation of S8 and S9 also significantly reduced the binding of ShcB to TrkA (Fig.  2 B,  top panel,  lane 6), which confirmed that Tyr499 is the binding site of ShcB to TrkA.	bind
40301	2	9489	7	NULL	NULL	0	NULL	 S8	NULL	mutation of	reduce	NULL	significantly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26046_s_210	12006576	A combination mutation of S8 and S9 also significantly reduced the binding of ShcB to TrkA (Fig.  2 B,  top panel,  lane 6), which confirmed that Tyr499 is the binding site of ShcB to TrkA.	bind
40302	3	9489	7	NULL	NULL	0	NULL	S9	NULL	mutation of	reduce	NULL	significantly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26046_s_210	12006576	A combination mutation of S8 and S9 also significantly reduced the binding of ShcB to TrkA (Fig.  2 B,  top panel,  lane 6), which confirmed that Tyr499 is the binding site of ShcB to TrkA.	bind
41352	1	9490	5	13	NULL	NULL	NULL	DNA complex	NucleicAcid	ATP-induced	consists		predominantly			NFAT-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_19_13205_s_210	10224077	A combination of anti-NFAT-1 and anti-NFAT-2 strongly prevented DNA binding, indicating that the ATP-induced DNA complex predominantly consisted of NFAT-1 and NFAT-2.	bind
41353	2	9490	5	13	NULL	NULL	NULL	DNA complex	NucleicAcid	ATP-induced	consists		predominantly			NFAT-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_19_13205_s_210	10224077	A combination of anti-NFAT-1 and anti-NFAT-2 strongly prevented DNA binding, indicating that the ATP-induced DNA complex predominantly consisted of NFAT-1 and NFAT-2.	bind
40303	1	9490	7	NULL	NULL	0	NULL	anti-NFAT-1 	NULL		prevents	NULL	strongly			DNA	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_19_13205_s_210	10224077	A combination of anti-NFAT-1 and anti-NFAT-2 strongly prevented DNA binding, indicating that the ATP-induced DNA complex predominantly consisted of NFAT-1 and NFAT-2.	bind
40304	2	9490	7	NULL	NULL	0	NULL	anti-NFAT-2	NULL		prevents	NULL	strongly			DNA	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_19_13205_s_210	10224077	A combination of anti-NFAT-1 and anti-NFAT-2 strongly prevented DNA binding, indicating that the ATP-induced DNA complex predominantly consisted of NFAT-1 and NFAT-2.	bind
40305	3	9490	7	NULL	NULL	0	NULL	statement 1	NULL		occur in combination with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_19_13205_s_210	10224077	A combination of anti-NFAT-1 and anti-NFAT-2 strongly prevented DNA binding, indicating that the ATP-induced DNA complex predominantly consisted of NFAT-1 and NFAT-2.	bind
40306	4	9490	7	NULL	NULL	0	NULL	ATP	NULL		induce	NULL				DNA complex	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_19_13205_s_210	10224077	A combination of anti-NFAT-1 and anti-NFAT-2 strongly prevented DNA binding, indicating that the ATP-induced DNA complex predominantly consisted of NFAT-1 and NFAT-2.	bind
40307	5	9490	7	NULL	NULL	0	NULL	statement 4	NULL		consist of	NULL				NFAT-1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_19_13205_s_210	10224077	A combination of anti-NFAT-1 and anti-NFAT-2 strongly prevented DNA binding, indicating that the ATP-induced DNA complex predominantly consisted of NFAT-1 and NFAT-2.	bind
40308	6	9490	7	NULL	NULL	0	NULL	statement 4	NULL		consist of	NULL				NFAT-2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_19_13205_s_210	10224077	A combination of anti-NFAT-1 and anti-NFAT-2 strongly prevented DNA binding, indicating that the ATP-induced DNA complex predominantly consisted of NFAT-1 and NFAT-2.	bind
41355	2	9492	5	13	NULL	NULL	NULL	secretory vesicles	CellComponent	small	depart from					trans-Golgi compartments	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_17_16868_s_23	15718243	A combination of mucin granules released at a very low rate and/or small secretory vesicles departing from the  trans-Golgi compartments might mediate constitutive mucin secretion ( ,  ).	bind
41356	3	9492	5	13	NULL	NULL	NULL	statement 2	Process		mediate					mucin	GP	constitutive secretion of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_17_16868_s_23	15718243	A combination of mucin granules released at a very low rate and/or small secretory vesicles departing from the  trans-Golgi compartments might mediate constitutive mucin secretion ( ,  ).	bind
56758	1	9492	5	13	NULL	NULL	NULL	mucin granules	CellComponent		mediate		might			mucin	GP	secretion of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_17_16868_s_23	15718243	A combination of mucin granules released at a very low rate and/or small secretory vesicles departing from the  trans-Golgi compartments might mediate constitutive mucin secretion ( ,  ).	bind
56762	4	9492	5	13	NULL	NULL	NULL	statement 1	Process		occur in combination of					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_17_16868_s_23	15718243	A combination of mucin granules released at a very low rate and/or small secretory vesicles departing from the  trans-Golgi compartments might mediate constitutive mucin secretion ( ,  ).	bind
56780	5	9492	5	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_17_16868_s_23	15718243	A combination of mucin granules released at a very low rate and/or small secretory vesicles departing from the  trans-Golgi compartments might mediate constitutive mucin secretion ( ,  ).	bind
40323	1	9492	7	NULL	NULL	0	NULL	mucin granules	NULL		mediate	NULL	might			mucin	NULL	secretion of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_17_16868_s_23	15718243	A combination of mucin granules released at a very low rate and/or small secretory vesicles departing from the  trans-Golgi compartments might mediate constitutive mucin secretion ( ,  ).	bind
40324	2	9492	7	NULL	NULL	0	NULL	small secretory vesicles	NULL		depart from	NULL				trans-Golgi compartments	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_17_16868_s_23	15718243	A combination of mucin granules released at a very low rate and/or small secretory vesicles departing from the  trans-Golgi compartments might mediate constitutive mucin secretion ( ,  ).	bind
40325	3	9492	7	NULL	NULL	0	NULL	statement 2	NULL		mediate	NULL	might			mucin	NULL	secretion of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_17_16868_s_23	15718243	A combination of mucin granules released at a very low rate and/or small secretory vesicles departing from the  trans-Golgi compartments might mediate constitutive mucin secretion ( ,  ).	bind
40326	4	9492	7	NULL	NULL	0	NULL	statement 1	NULL		occur in combination with	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_17_16868_s_23	15718243	A combination of mucin granules released at a very low rate and/or small secretory vesicles departing from the  trans-Golgi compartments might mediate constitutive mucin secretion ( ,  ).	bind
40327	5	9492	7	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_17_16868_s_23	15718243	A combination of mucin granules released at a very low rate and/or small secretory vesicles departing from the  trans-Golgi compartments might mediate constitutive mucin secretion ( ,  ).	bind
41357	1	9493	5	13	NULL	NULL	NULL	GST-AGS3	GP		bind					Galphai	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_9_6767_s_97	11756403	A combination of the inactive GPR truncation peptides (GPR 1-15 and GPR 15-28) did not inhibit binding of GST-AGS3 to Galphai.	bind
41358	2	9493	5	13	NULL	NULL	NULL	GPR	GP		does not inhibit			1-15		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_9_6767_s_97	11756403	A combination of the inactive GPR truncation peptides (GPR 1-15 and GPR 15-28) did not inhibit binding of GST-AGS3 to Galphai.	bind
41359	3	9493	5	13	NULL	NULL	NULL	GPR	GP		does not inhibit			15-28		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_9_6767_s_97	11756403	A combination of the inactive GPR truncation peptides (GPR 1-15 and GPR 15-28) did not inhibit binding of GST-AGS3 to Galphai.	bind
41360	4	9493	5	13	NULL	NULL	NULL	GPR	GP	inactive 	is			1-15		GPR truncation peptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_9_6767_s_97	11756403	A combination of the inactive GPR truncation peptides (GPR 1-15 and GPR 15-28) did not inhibit binding of GST-AGS3 to Galphai.	bind
41361	5	9493	5	13	NULL	NULL	NULL	GPR	GP	inactive	is			15-28		GPR truncation peptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_9_6767_s_97	11756403	A combination of the inactive GPR truncation peptides (GPR 1-15 and GPR 15-28) did not inhibit binding of GST-AGS3 to Galphai.	bind
40328	1	9493	7	NULL	NULL	0	NULL	GST-AGS3	NULL		bind	NULL				Galphai	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_9_6767_s_97	11756403	A combination of the inactive GPR truncation peptides (GPR 1-15 and GPR 15-28) did not inhibit binding of GST-AGS3 to Galphai.	bind
40329	2	9493	7	NULL	NULL	0	NULL	GPR 1-15	NULL	inactive	does not inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_9_6767_s_97	11756403	A combination of the inactive GPR truncation peptides (GPR 1-15 and GPR 15-28) did not inhibit binding of GST-AGS3 to Galphai.	bind
40330	3	9493	7	NULL	NULL	0	NULL	GPR 15-28	NULL	inactive	does not inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_9_6767_s_97	11756403	A combination of the inactive GPR truncation peptides (GPR 1-15 and GPR 15-28) did not inhibit binding of GST-AGS3 to Galphai.	bind
40331	4	9493	7	NULL	NULL	0	NULL	GPR 1-15	NULL		is a type of	NULL				GPR truncation peptides	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_9_6767_s_97	11756403	A combination of the inactive GPR truncation peptides (GPR 1-15 and GPR 15-28) did not inhibit binding of GST-AGS3 to Galphai.	bind
40332	5	9493	7	NULL	NULL	0	NULL	GPR 15-28	NULL		is a type of	NULL				GPR truncation peptides	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_9_6767_s_97	11756403	A combination of the inactive GPR truncation peptides (GPR 1-15 and GPR 15-28) did not inhibit binding of GST-AGS3 to Galphai.	bind
41362	1	9494	5	13	NULL	NULL	NULL			combined mutation	decrease		selectively	Y13L/S14Q		IL8R2	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_14_8228_s_13	8626516	A combined  mutation Y13L/S14Q selectively decreased binding to IL8R2.	bind
40333	1	9494	7	10	NULL	0	NULL		NULL	combined mutation	decrease	NULL	selectively	Y13L/S14Q		IL8R2	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_14_8228_s_13	8626516	A combined  mutation Y13L/S14Q selectively decreased binding to IL8R2.	bind
41602	1	9495	5	13	NULL	NULL	NULL	Smad3	GP		bind					p300	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_14_2114_s_51	9679056	A combined amino- and carboxy-terminal truncation (210-342) bound to p300 comparably as well as the 2-342 and 210-425 molecules, indicating that the carboxyl and amino termini of Smad3 can only negatively regulate binding of Smad3 to p300 when the other terminus is still present.	bind
41616	2	9495	5	13	NULL	NULL	NULL	Smad3	GP	truncated	bind			2-342		p300	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_14_2114_s_51	9679056	A combined amino- and carboxy-terminal truncation (210-342) bound to p300 comparably as well as the 2-342 and 210-425 molecules, indicating that the carboxyl and amino termini of Smad3 can only negatively regulate binding of Smad3 to p300 when the other terminus is still present.	bind
41617	3	9495	5	13	NULL	NULL	NULL	Smad3	GP	truncated	bind			210-425		p300	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_14_2114_s_51	9679056	A combined amino- and carboxy-terminal truncation (210-342) bound to p300 comparably as well as the 2-342 and 210-425 molecules, indicating that the carboxyl and amino termini of Smad3 can only negatively regulate binding of Smad3 to p300 when the other terminus is still present.	bind
41618	4	9495	5	13	NULL	NULL	NULL	Smad3	GP	truncated	bind			210-342		p300	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_14_2114_s_51	9679056	A combined amino- and carboxy-terminal truncation (210-342) bound to p300 comparably as well as the 2-342 and 210-425 molecules, indicating that the carboxyl and amino termini of Smad3 can only negatively regulate binding of Smad3 to p300 when the other terminus is still present.	bind
41619	5	9495	5	13	NULL	NULL	NULL	Smad3	GP	truncated	is			210-342		combined amino- and carboxy-terminal truncation of Smad3	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_14_2114_s_51	9679056	A combined amino- and carboxy-terminal truncation (210-342) bound to p300 comparably as well as the 2-342 and 210-425 molecules, indicating that the carboxyl and amino termini of Smad3 can only negatively regulate binding of Smad3 to p300 when the other terminus is still present.	bind
41620	6	9495	5	13	NULL	NULL	NULL	Smad3	GP		regulates		negatively	carboxyl & amino termini		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_14_2114_s_51	9679056	A combined amino- and carboxy-terminal truncation (210-342) bound to p300 comparably as well as the 2-342 and 210-425 molecules, indicating that the carboxyl and amino termini of Smad3 can only negatively regulate binding of Smad3 to p300 when the other terminus is still present.	bind
40334	1	9495	7	NULL	NULL	0	NULL	 Smad3	NULL		bind	NULL				p300	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_14_2114_s_51	9679056	A combined amino- and carboxy-terminal truncation (210-342) bound to p300 comparably as well as the 2-342 and 210-425 molecules, indicating that the carboxyl and amino termini of Smad3 can only negatively regulate binding of Smad3 to p300 when the other terminus is still present.	bind
40335	2	9495	7	10	NULL	0	NULL	Smad3	NULL	truncated	bind	NULL		amino- and carboxy-terminal		p300	NULL				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_14_2114_s_51	9679056	A combined amino- and carboxy-terminal truncation (210-342) bound to p300 comparably as well as the 2-342 and 210-425 molecules, indicating that the carboxyl and amino termini of Smad3 can only negatively regulate binding of Smad3 to p300 when the other terminus is still present.	bind
40336	3	9495	7	10	NULL	0	NULL	Smad3	NULL	truncated	bind	NULL		 2-342 molecule		p300	NULL				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_14_2114_s_51	9679056	A combined amino- and carboxy-terminal truncation (210-342) bound to p300 comparably as well as the 2-342 and 210-425 molecules, indicating that the carboxyl and amino termini of Smad3 can only negatively regulate binding of Smad3 to p300 when the other terminus is still present.	bind
40337	4	9495	7	10	NULL	0	NULL	Smad3	NULL	truncated	bind	NULL		210-425 molecule		p300	NULL				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_14_2114_s_51	9679056	A combined amino- and carboxy-terminal truncation (210-342) bound to p300 comparably as well as the 2-342 and 210-425 molecules, indicating that the carboxyl and amino termini of Smad3 can only negatively regulate binding of Smad3 to p300 when the other terminus is still present.	bind
40338	5	9495	7	NULL	NULL	0	NULL	Smad3	NULL		regulate	NULL	negatively	 carboxyl and amino termini		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_14_2114_s_51	9679056	A combined amino- and carboxy-terminal truncation (210-342) bound to p300 comparably as well as the 2-342 and 210-425 molecules, indicating that the carboxyl and amino termini of Smad3 can only negatively regulate binding of Smad3 to p300 when the other terminus is still present.	bind
41363	1	9496	5	13	NULL	NULL	NULL	67 kDa protein	GP		is a type of					calmodulin binding protein	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_gut_32_10_1955165_s_4	1955165	A common  calmodulin binding protein of 67 kDa was found in membrane and cytosolic  fractions of oesophagus, stomach, proximal and distal small intestine,  and colon from all four species.	bind
41364	2	9496	5	13	NULL	NULL	NULL	67 kDa protein	GP		is present in					oesophagus	OrganismPart	membrane fractions of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_gut_32_10_1955165_s_4	1955165	A common  calmodulin binding protein of 67 kDa was found in membrane and cytosolic  fractions of oesophagus, stomach, proximal and distal small intestine,  and colon from all four species.	bind
41365	3	9496	5	13	NULL	NULL	NULL	67 kDa protein	GP		is present in					stomach	OrganismPart	membrane fractions of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_gut_32_10_1955165_s_4	1955165	A common  calmodulin binding protein of 67 kDa was found in membrane and cytosolic  fractions of oesophagus, stomach, proximal and distal small intestine,  and colon from all four species.	bind
41366	4	9496	5	13	NULL	NULL	NULL	67 kDa protein	GP		is present in					proximal small intestine	OrganismPart	membrane fractions of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_gut_32_10_1955165_s_4	1955165	A common  calmodulin binding protein of 67 kDa was found in membrane and cytosolic  fractions of oesophagus, stomach, proximal and distal small intestine,  and colon from all four species.	bind
41367	5	9496	5	13	NULL	NULL	NULL	67 kDa protein	GP		is present in					distal small intestine	OrganismPart	membrane fractions of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_gut_32_10_1955165_s_4	1955165	A common  calmodulin binding protein of 67 kDa was found in membrane and cytosolic  fractions of oesophagus, stomach, proximal and distal small intestine,  and colon from all four species.	bind
41368	6	9496	5	13	NULL	NULL	NULL	67 kDa protein	GP		is present in					colon	OrganismPart	membrane fractions of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_gut_32_10_1955165_s_4	1955165	A common  calmodulin binding protein of 67 kDa was found in membrane and cytosolic  fractions of oesophagus, stomach, proximal and distal small intestine,  and colon from all four species.	bind
41369	7	9496	5	13	NULL	NULL	NULL	67 kDa protein	GP		is present in					oesophagus	OrganismPart	cytosolic fractions of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_gut_32_10_1955165_s_4	1955165	A common  calmodulin binding protein of 67 kDa was found in membrane and cytosolic  fractions of oesophagus, stomach, proximal and distal small intestine,  and colon from all four species.	bind
41370	8	9496	5	13	NULL	NULL	NULL	67 kDa protein	GP		is present in					stomach	OrganismPart	cytosolic fractions of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_gut_32_10_1955165_s_4	1955165	A common  calmodulin binding protein of 67 kDa was found in membrane and cytosolic  fractions of oesophagus, stomach, proximal and distal small intestine,  and colon from all four species.	bind
41371	9	9496	5	13	NULL	NULL	NULL	67 kDa protein	GP		is present in					proximal small intestine	OrganismPart	cytosolic fractions of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_gut_32_10_1955165_s_4	1955165	A common  calmodulin binding protein of 67 kDa was found in membrane and cytosolic  fractions of oesophagus, stomach, proximal and distal small intestine,  and colon from all four species.	bind
41372	10	9496	5	13	NULL	NULL	NULL	67 kDa protein	GP		is present in					distal small intestine	OrganismPart	cytosolic fractions of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_gut_32_10_1955165_s_4	1955165	A common  calmodulin binding protein of 67 kDa was found in membrane and cytosolic  fractions of oesophagus, stomach, proximal and distal small intestine,  and colon from all four species.	bind
41373	11	9496	5	13	NULL	NULL	NULL	67 kDa protein	GP		is present in					colon	GP	cytosolic fractions of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_gut_32_10_1955165_s_4	1955165	A common  calmodulin binding protein of 67 kDa was found in membrane and cytosolic  fractions of oesophagus, stomach, proximal and distal small intestine,  and colon from all four species.	bind
40339	1	9496	7	NULL	NULL	0	NULL	 67 kDa protein	NULL		is found in	NULL				 oesophagus	NULL	membrane fractions of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_gut_32_10_1955165_s_4	1955165	A common  calmodulin binding protein of 67 kDa was found in membrane and cytosolic  fractions of oesophagus, stomach, proximal and distal small intestine,  and colon from all four species.	bind
40340	2	9496	7	NULL	NULL	0	NULL	67kDa  protein	NULL		is found in	NULL				stomach	NULL	membrane fractions of 			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_gut_32_10_1955165_s_4	1955165	A common  calmodulin binding protein of 67 kDa was found in membrane and cytosolic  fractions of oesophagus, stomach, proximal and distal small intestine,  and colon from all four species.	bind
40341	3	9496	7	NULL	NULL	0	NULL	67 kDa  protein	NULL		is found in	NULL				colon	NULL	membrane fractions of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_gut_32_10_1955165_s_4	1955165	A common  calmodulin binding protein of 67 kDa was found in membrane and cytosolic  fractions of oesophagus, stomach, proximal and distal small intestine,  and colon from all four species.	bind
40342	4	9496	7	NULL	NULL	0	NULL	67kDa  protein	NULL		is found in	NULL				proximal small intestine	NULL	membrane fractions of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_gut_32_10_1955165_s_4	1955165	A common  calmodulin binding protein of 67 kDa was found in membrane and cytosolic  fractions of oesophagus, stomach, proximal and distal small intestine,  and colon from all four species.	bind
40343	5	9496	7	NULL	NULL	0	NULL	67kDa  protein	NULL		is found in	NULL				distal small intestine	NULL	membrane fractions of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_gut_32_10_1955165_s_4	1955165	A common  calmodulin binding protein of 67 kDa was found in membrane and cytosolic  fractions of oesophagus, stomach, proximal and distal small intestine,  and colon from all four species.	bind
40344	6	9496	7	NULL	NULL	0	NULL	67kDa  protein	NULL		is found in	NULL				stomach	NULL	cytosolic fractions of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_gut_32_10_1955165_s_4	1955165	A common  calmodulin binding protein of 67 kDa was found in membrane and cytosolic  fractions of oesophagus, stomach, proximal and distal small intestine,  and colon from all four species.	bind
46968	7	9496	7	NULL	NULL	0	NULL	67 kDa  protein	NULL		is found in	NULL				 oesophagus	NULL	cytosolic fractions of			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_gut_32_10_1955165_s_4	1955165	A common  calmodulin binding protein of 67 kDa was found in membrane and cytosolic  fractions of oesophagus, stomach, proximal and distal small intestine,  and colon from all four species.	bind
46969	8	9496	7	NULL	NULL	0	NULL	67kDa  protein	NULL		is found in	NULL				proximal small intestine	NULL	cytosolic fractions of			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_gut_32_10_1955165_s_4	1955165	A common  calmodulin binding protein of 67 kDa was found in membrane and cytosolic  fractions of oesophagus, stomach, proximal and distal small intestine,  and colon from all four species.	bind
46970	9	9496	7	NULL	NULL	0	NULL	67kDa  protein	NULL		is found in	NULL				distal small intestine	NULL	cytosolic fractions of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_gut_32_10_1955165_s_4	1955165	A common  calmodulin binding protein of 67 kDa was found in membrane and cytosolic  fractions of oesophagus, stomach, proximal and distal small intestine,  and colon from all four species.	bind
46971	10	9496	7	NULL	NULL	0	NULL	67kDa  protein	NULL		is found in	NULL				colon	NULL	cytosolic fractions of			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_gut_32_10_1955165_s_4	1955165	A common  calmodulin binding protein of 67 kDa was found in membrane and cytosolic  fractions of oesophagus, stomach, proximal and distal small intestine,  and colon from all four species.	bind
46972	11	9496	7	NULL	NULL	0	NULL	67kDa  protein	NULL		is a type of	NULL				calmodulin binding protein	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_gut_32_10_1955165_s_4	1955165	A common  calmodulin binding protein of 67 kDa was found in membrane and cytosolic  fractions of oesophagus, stomach, proximal and distal small intestine,  and colon from all four species.	bind
41670	1	9497	5	13	NULL	NULL	NULL	PEA-15	GP		is similar to			ERK-binding surface		Tube	GP		ERK-binding surface		NULL		NULL	NULL	NULL	NULL	gw60_embo_21_23_6494_s_138	12456656	A common binding surface in the death motif mediates diverse protein - protein interactions   A comparison of the ERK-binding surface of PEA-15 with that observed for Tube DD in the crystal structure of the Tube - Pelle DD complex ( Xiao  et al., 1999) revealed an unexpected similarity in the binding motifs of Tube and PEA-15 (Figure  6).	bind
40345	1	9497	7	NULL	NULL	0	NULL	PEA-15	NULL		is similar to	NULL		ERK-binding surface		Tube	NULL		binding motifs of		NULL		0	NULL	NULL	NULL	gw60_embo_21_23_6494_s_138	12456656	A common binding surface in the death motif mediates diverse protein - protein interactions   A comparison of the ERK-binding surface of PEA-15 with that observed for Tube DD in the crystal structure of the Tube - Pelle DD complex ( Xiao  et al., 1999) revealed an unexpected similarity in the binding motifs of Tube and PEA-15 (Figure  6).	bind
41374	1	9498	5	13	NULL	NULL	NULL	Hsc70	GP		plays a role in					TfR	GP	externalization of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_13_9910_s_263	11133993	A common explanation of the role of Hsc70 in TfR externalization is that after many rounds of endocytic cycles, along with changes in the cytoplasm during cell maturation, partial unfolding of the TfR cytoplasmic domain would expose the hydrophobic sequence that would bind Hsc70.	bind
41375	2	9498	5	13	NULL	NULL	NULL	TfR	GP		is exposed by			hydrophobic sequence		TfR	GP	partial unfolding of	cytoplasmic domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_13_9910_s_263	11133993	A common explanation of the role of Hsc70 in TfR externalization is that after many rounds of endocytic cycles, along with changes in the cytoplasm during cell maturation, partial unfolding of the TfR cytoplasmic domain would expose the hydrophobic sequence that would bind Hsc70.	bind
41376	3	9498	5	13	NULL	NULL	NULL	statement 2	GP		bind					Hsc70	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_13_9910_s_263	11133993	A common explanation of the role of Hsc70 in TfR externalization is that after many rounds of endocytic cycles, along with changes in the cytoplasm during cell maturation, partial unfolding of the TfR cytoplasmic domain would expose the hydrophobic sequence that would bind Hsc70.	bind
41377	4	9498	5	13	NULL	NULL	NULL	statement 3	Process		occurs during					cell maturation	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_13_9910_s_263	11133993	A common explanation of the role of Hsc70 in TfR externalization is that after many rounds of endocytic cycles, along with changes in the cytoplasm during cell maturation, partial unfolding of the TfR cytoplasmic domain would expose the hydrophobic sequence that would bind Hsc70.	bind
41378	5	9498	5	13	NULL	NULL	NULL	statement 4	Process		along with					cytoplasm	CellComponent	changes in			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_13_9910_s_263	11133993	A common explanation of the role of Hsc70 in TfR externalization is that after many rounds of endocytic cycles, along with changes in the cytoplasm during cell maturation, partial unfolding of the TfR cytoplasmic domain would expose the hydrophobic sequence that would bind Hsc70.	bind
41379	6	9498	5	13	NULL	NULL	NULL	statement 3	Process		occurs after					endocytic cycles	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_13_9910_s_263	11133993	A common explanation of the role of Hsc70 in TfR externalization is that after many rounds of endocytic cycles, along with changes in the cytoplasm during cell maturation, partial unfolding of the TfR cytoplasmic domain would expose the hydrophobic sequence that would bind Hsc70.	bind
40346	5	9498	7	NULL	NULL	0	NULL	statement 4	NULL		bind	NULL				Hsc 70	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_13_9910_s_263	11133993	A common explanation of the role of Hsc70 in TfR externalization is that after many rounds of endocytic cycles, along with changes in the cytoplasm during cell maturation, partial unfolding of the TfR cytoplasmic domain would expose the hydrophobic sequence that would bind Hsc70.	bind
48783	1	9498	7	NULL	NULL	0	NULL	Hsc70	NULL		plays a role in	NULL				TfR	NULL	externalization of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_13_9910_s_263	11133993	A common explanation of the role of Hsc70 in TfR externalization is that after many rounds of endocytic cycles, along with changes in the cytoplasm during cell maturation, partial unfolding of the TfR cytoplasmic domain would expose the hydrophobic sequence that would bind Hsc70.	bind
48784	2	9498	7	NULL	NULL	0	NULL	statement 1	NULL		occurs after	NULL				endocytic cycles	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_13_9910_s_263	11133993	A common explanation of the role of Hsc70 in TfR externalization is that after many rounds of endocytic cycles, along with changes in the cytoplasm during cell maturation, partial unfolding of the TfR cytoplasmic domain would expose the hydrophobic sequence that would bind Hsc70.	bind
48785	3	9498	7	NULL	NULL	0	NULL	statement 1	NULL		occurs during	NULL				cell maturation	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_13_9910_s_263	11133993	A common explanation of the role of Hsc70 in TfR externalization is that after many rounds of endocytic cycles, along with changes in the cytoplasm during cell maturation, partial unfolding of the TfR cytoplasmic domain would expose the hydrophobic sequence that would bind Hsc70.	bind
48786	4	9498	7	NULL	NULL	0	NULL	TfR 	NULL	partial unfolding of 	expose	NULL		cytoplasmic domain		hydrophobic sequence	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_13_9910_s_263	11133993	A common explanation of the role of Hsc70 in TfR externalization is that after many rounds of endocytic cycles, along with changes in the cytoplasm during cell maturation, partial unfolding of the TfR cytoplasmic domain would expose the hydrophobic sequence that would bind Hsc70.	bind
41380	1	9499	5	13	NULL	NULL	NULL	Ran	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40163_s_102	11024021	A common feature of nuclear transport receptors belonging to the importin beta family is their ability to specifically interact with the GTP-bound form of the small GTPase Ran.	bind
41381	2	9499	5	13	NULL	NULL	NULL	Ran	GP		is a type of					small GTPase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40163_s_102	11024021	A common feature of nuclear transport receptors belonging to the importin beta family is their ability to specifically interact with the GTP-bound form of the small GTPase Ran.	bind
41382	3	9499	5	13	NULL	NULL	NULL	nuclear transport receptors	GP		belong to					importin beta family	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40163_s_102	11024021	A common feature of nuclear transport receptors belonging to the importin beta family is their ability to specifically interact with the GTP-bound form of the small GTPase Ran.	bind
41383	4	9499	5	13	NULL	NULL	NULL	nuclear transport receptor	GP		interact with					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40163_s_102	11024021	A common feature of nuclear transport receptors belonging to the importin beta family is their ability to specifically interact with the GTP-bound form of the small GTPase Ran.	bind
40347	1	9499	7	10	NULL	0	NULL	GTP	NULL		bind	NULL				Ran	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40163_s_102	11024021	A common feature of nuclear transport receptors belonging to the importin beta family is their ability to specifically interact with the GTP-bound form of the small GTPase Ran.	bind
40348	2	9499	7	NULL	NULL	0	NULL	nuclear transport receptors 	NULL		belongs to	NULL				importin beta family	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_51_40163_s_102	11024021	A common feature of nuclear transport receptors belonging to the importin beta family is their ability to specifically interact with the GTP-bound form of the small GTPase Ran.	bind
40349	3	9499	7	NULL	NULL	0	NULL	Ran	NULL		is a type of	NULL				small GTPase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_51_40163_s_102	11024021	A common feature of nuclear transport receptors belonging to the importin beta family is their ability to specifically interact with the GTP-bound form of the small GTPase Ran.	bind
46845	4	9499	7	10	NULL	0	NULL	nuclear transport receptors	NULL		bind	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_51_40163_s_102	11024021	A common feature of nuclear transport receptors belonging to the importin beta family is their ability to specifically interact with the GTP-bound form of the small GTPase Ran.	bind
41384	1	9500	5	13	NULL	NULL	NULL	b12	GP		bind					gp120	GP				NULL	clade B isolates	NULL	NULL	NULL	NULL	gw60_science_293_5532_1155_s_132	11498595	A common feature of these neutralization escape variants is the mutation of a proline at position 369, which strongly reduces b12 binding to gp120 in clade B isolates ( 50).	bind
41386	2	9500	5	13	NULL	NULL	NULL			mutation of	reduce		strongly	proline 369		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_293_5532_1155_s_132	11498595	A common feature of these neutralization escape variants is the mutation of a proline at position 369, which strongly reduces b12 binding to gp120 in clade B isolates ( 50).	bind
40350	1	9500	7	NULL	NULL	0	NULL	b12	NULL		bind	NULL				gp120	NULL				NULL	clade B isolates	0	NULL	NULL	NULL	gw60_science_293_5532_1155_s_132	11498595	A common feature of these neutralization escape variants is the mutation of a proline at position 369, which strongly reduces b12 binding to gp120 in clade B isolates ( 50).	bind
40351	2	9500	7	NULL	NULL	0	NULL		NULL	mutation of	reduce	NULL	strongly	proline 369		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_science_293_5532_1155_s_132	11498595	A common feature of these neutralization escape variants is the mutation of a proline at position 369, which strongly reduces b12 binding to gp120 in clade B isolates ( 50).	bind
41387	1	9502	5	13	NULL	NULL	NULL	MSL proteins	GP		bind					roX RNAs	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_269_1_18_s_105	15081354	A common point of confusion arises from the fact that MSL proteins bind to both  roX RNAs and  roX genes.	bind
41388	2	9502	5	13	NULL	NULL	NULL	MSL proteins	GP		bind					roX genes	GP				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_269_1_18_s_105	15081354	A common point of confusion arises from the fact that MSL proteins bind to both  roX RNAs and  roX genes.	bind
40352	1	9502	7	NULL	NULL	0	NULL	MSL protein	NULL		bind	NULL				roX RNAs	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_269_1_18_s_105	15081354	A common point of confusion arises from the fact that MSL proteins bind to both  roX RNAs and  roX genes.	bind
40353	2	9502	7	NULL	NULL	0	NULL	MSL protein	NULL		bind	NULL				 roX gene	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_269_1_18_s_105	15081354	A common point of confusion arises from the fact that MSL proteins bind to both  roX RNAs and  roX genes.	bind
41389	1	9503	5	13	NULL	NULL	NULL	P-gp	GP		bind					vinblastine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_58_3_624_s_104	10953057	A common property of these modulators is the ability to reduce the maximal binding capacity of P-gp for [3]vinblastine (Fig.  1).	bind
40354	1	9503	7	NULL	NULL	0	NULL	P-gp	NULL		bind	NULL				vinblastine	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_58_3_624_s_104	10953057	A common property of these modulators is the ability to reduce the maximal binding capacity of P-gp for [3]vinblastine (Fig.  1).	bind
41391	1	9504	5	13	NULL	NULL	NULL	p300	GP		bind					Cdk protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_57	10330164	A common region of p300 binds to Cdk, TFIIB, and E1A proteins.	bind
41392	2	9504	5	13	NULL	NULL	NULL	p300	GP		bind					TFIIB protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_57	10330164	A common region of p300 binds to Cdk, TFIIB, and E1A proteins.	bind
41393	3	9504	5	13	NULL	NULL	NULL	p300	GP		bind					E1A protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_57	10330164	A common region of p300 binds to Cdk, TFIIB, and E1A proteins.	bind
40355	1	9504	7	NULL	NULL	0	NULL	p300	NULL		binds to	NULL				Cdk protein	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_57	10330164	A common region of p300 binds to Cdk, TFIIB, and E1A proteins.	bind
40356	2	9504	7	NULL	NULL	0	NULL	p300	NULL		binds to	NULL				TFIIB protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_57	10330164	A common region of p300 binds to Cdk, TFIIB, and E1A proteins.	bind
40357	3	9504	7	NULL	NULL	0	NULL	p300	NULL		binds to	NULL				E1A protein	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_6_4241_s_57	10330164	A common region of p300 binds to Cdk, TFIIB, and E1A proteins.	bind
41394	1	9506	5	13	NULL	NULL	NULL	virulence factors	GP		bind					secretion chaperones	GP	bacterial			NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_mol-cell_21_5_16507363_s_1	16507363	A common structural motif in the binding of virulence factors to bacterial secretion chaperones..	bind
40358	1	9506	7	10	NULL	0	NULL	virulence factors	NULL		bind	NULL				secretion chaperones	NULL	bacterial 			NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_mol-cell_21_5_16507363_s_1	16507363	A common structural motif in the binding of virulence factors to bacterial secretion chaperones..	bind
41395	1	9507	5	13	NULL	NULL	NULL	[35]-GTP gammaS	GP		bind					Gq alpha	GP				NULL	CHO-m2m3 membranes	NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_7_1340_s_80	12711635	A comparable increase in [35]-GTP gammaS binding to Gq alpha was observed in CHO-m2m3 membranes and MCh stimulated this response with similar potencies in the two preparations (pEC50 values: CHO-m3, 4.49 plus-or-minus 0.34; CHO-m2m3, 4.29 plus-or-minus 0.37).	bind
40359	1	9507	7	NULL	NULL	0	NULL	[35]-GTP gammaS	NULL		bind	NULL				Gq alpha	NULL				NULL	CHO-m2m3 membranes	0	NULL	NULL	NULL	gw60_brjpharmacol_138_7_1340_s_80	12711635	A comparable increase in [35]-GTP gammaS binding to Gq alpha was observed in CHO-m2m3 membranes and MCh stimulated this response with similar potencies in the two preparations (pEC50 values: CHO-m3, 4.49 plus-or-minus 0.34; CHO-m2m3, 4.29 plus-or-minus 0.37).	bind
41397	1	9508	5	13	NULL	NULL	NULL	RecA	GP	mutation of	bind			K72R		ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31397_s_313	8537414	A comparable mutation in the conserved ATP  binding site of the RecA protein (RecA K72R) creates an altered protein  that binds, but does not hydrolyze ATP( 38) .	bind
41399	2	9508	5	13	NULL	NULL	NULL	statement 1	Process		does not hydrolyze					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31397_s_313	8537414	A comparable mutation in the conserved ATP  binding site of the RecA protein (RecA K72R) creates an altered protein  that binds, but does not hydrolyze ATP( 38) .	bind
40360	1	9508	7	10	NULL	0	NULL	RecA		 mutation of	bind			K72R		ATP					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31397_s_313	8537414	A comparable mutation in the conserved ATP  binding site of the RecA protein (RecA K72R) creates an altered protein  that binds, but does not hydrolyze ATP( 38) .	bind
40361	2	9508	7	NULL	NULL	0	NULL	statement 1	NULL		does not hydrolyse	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31397_s_313	8537414	A comparable mutation in the conserved ATP  binding site of the RecA protein (RecA K72R) creates an altered protein  that binds, but does not hydrolyze ATP( 38) .	bind
41400	1	9509	5	13	NULL	NULL	NULL	p53	GP		bind					PCNA gene	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_45_44009_s_229	12947108	A comparable, yet distinct, profile of p53 binding to the PCNA gene was observed in the ChIP assay.	bind
40362	1	9509	7	NULL	NULL	0	NULL	p53	NULL		bind	NULL				PCNA gene	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_45_44009_s_229	12947108	A comparable, yet distinct, profile of p53 binding to the PCNA gene was observed in the ChIP assay.	bind
41674	1	9510	5	13	NULL	NULL	NULL	E2 protein	GP		bind		high affinity;;sequence-specific			DNA	NucleicAcid			A-tract structure of the core region	NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_15_8490_s_4	11438706	A comparative analysis of E2-DNA conformations with respect to other structural and biochemical studies demonstrates that ( i) the A-tract structure of the core region, which is not contacted by the protein, is critical for the formation of the high-affinity sequence-specific protein-DNA complex, and ( ii) differential binding affinity is regulated by the intrinsic structure and deformability encoded in the base sequence of the DNA target.	bind
42380	2	9510	5	13	NULL	NULL	NULL				is critical for				A-tract structure of the core region	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_15_8490_s_4	11438706	A comparative analysis of E2-DNA conformations with respect to other structural and biochemical studies demonstrates that ( i) the A-tract structure of the core region, which is not contacted by the protein, is critical for the formation of the high-affinity sequence-specific protein-DNA complex, and ( ii) differential binding affinity is regulated by the intrinsic structure and deformability encoded in the base sequence of the DNA target.	bind
40363	1	9510	7	10	NULL	0	NULL	E2 protein			complex with		high affinity;;sequence specific			DNA				A-tract structure of the core region	NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_15_8490_s_4	11438706	A comparative analysis of E2-DNA conformations with respect to other structural and biochemical studies demonstrates that ( i) the A-tract structure of the core region, which is not contacted by the protein, is critical for the formation of the high-affinity sequence-specific protein-DNA complex, and ( ii) differential binding affinity is regulated by the intrinsic structure and deformability encoded in the base sequence of the DNA target.	bind
40364	2	9510	7	10	NULL	0	NULL	A-tract structure			is critical for			core region		statement 1					NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_15_8490_s_4	11438706	A comparative analysis of E2-DNA conformations with respect to other structural and biochemical studies demonstrates that ( i) the A-tract structure of the core region, which is not contacted by the protein, is critical for the formation of the high-affinity sequence-specific protein-DNA complex, and ( ii) differential binding affinity is regulated by the intrinsic structure and deformability encoded in the base sequence of the DNA target.	bind
41401	1	9512	5	13	NULL	NULL	NULL	MBD proteins	GP	multiple	bind					hypermethylated genes	GP	cancer-associated			NULL	human cancer cell lines	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_13_4243_s_33	16052033	A comparative study in human cancer cell lines using a chromatin immunoprecipitation (ChIP) assay combined with a CpG island microarray also suggests some specificities, since some cancer-associated hypermethylated genes are bound by multiple MBD proteins while others are associated with a single MBD protein ( ).	bind
56789	2	9512	5	13	NULL	NULL	NULL	MBD protein	GP	single	bind					hypermethylated genes	GP	cancer-associated			NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_13_4243_s_33	16052033	A comparative study in human cancer cell lines using a chromatin immunoprecipitation (ChIP) assay combined with a CpG island microarray also suggests some specificities, since some cancer-associated hypermethylated genes are bound by multiple MBD proteins while others are associated with a single MBD protein ( ).	bind
40440	1	9512	7	10	NULL	0	NULL	MBD proteins		multiple	bind					hypermethylated genes 		cancer-associated 			NULL	human cancer cell lines	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_13_4243_s_33	16052033	A comparative study in human cancer cell lines using a chromatin immunoprecipitation (ChIP) assay combined with a CpG island microarray also suggests some specificities, since some cancer-associated hypermethylated genes are bound by multiple MBD proteins while others are associated with a single MBD protein ( ).	bind
40442	2	9512	7	10	NULL	0	NULL	MBD protein		single	bind					hypermethylated genes		cancer-associated 			NULL	human cancer cell lines	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_13_4243_s_33	16052033	A comparative study in human cancer cell lines using a chromatin immunoprecipitation (ChIP) assay combined with a CpG island microarray also suggests some specificities, since some cancer-associated hypermethylated genes are bound by multiple MBD proteins while others are associated with a single MBD protein ( ).	bind
41402	1	9513	5	13	NULL	NULL	NULL	Azide	Chemical		bind					amine oxidases	GP	copper-containing			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_biochemistry_45_29_16846222_s_1	16846222	A Comparative Study of the Binding and Inhibition of Four Copper-Containing Amine Oxidases by Azide:	bind
41403	2	9513	5	13	NULL	NULL	NULL	statement 1	Chemical		inhibit					amine oxidases	GP	copper-containing			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_biochemistry_45_29_16846222_s_1	16846222	A Comparative Study of the Binding and Inhibition of Four Copper-Containing Amine Oxidases by Azide:	bind
40452	1	9513	7	10	NULL	0	NULL	Azide			bind					Amine Oxidase		Copper-Containing 			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_biochemistry_45_29_16846222_s_1	16846222	A Comparative Study of the Binding and Inhibition of Four Copper-Containing Amine Oxidases by Azide:	bind
40453	2	9513	7	10	NULL	0	NULL	statement 1			inhibit					Amine Oxidase		Copper-Containing			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_biochemistry_45_29_16846222_s_1	16846222	A Comparative Study of the Binding and Inhibition of Four Copper-Containing Amine Oxidases by Azide:	bind
41404	1	9514	5	13	NULL	NULL	NULL	MT1	GP		bind					MMP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_13_11201_s_44	11790786	A comparative study of these compounds on the activation of pro-MMP-2 in cells expressing MT1-MMP shows that, when compared with marimastat, significantly higher dithiol concentrations are required for active MT1-MMP binding and enhancement of pro-MMP-2 activation in the presence of TIMP-2.	bind
41405	2	9514	5	13	NULL	NULL	NULL	marimastat	Chemical		is required for					MT1-MMP	GP	binding of active			NULL	cells expressing MT1-MMP	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_13_11201_s_44	11790786	A comparative study of these compounds on the activation of pro-MMP-2 in cells expressing MT1-MMP shows that, when compared with marimastat, significantly higher dithiol concentrations are required for active MT1-MMP binding and enhancement of pro-MMP-2 activation in the presence of TIMP-2.	bind
41406	3	9514	5	13	NULL	NULL	NULL	marimastat	Chemical		is required for					pro-MMP-2	GP	enhancement of;;activation of			NULL	cells expressing MT1-MMP	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_13_11201_s_44	11790786	A comparative study of these compounds on the activation of pro-MMP-2 in cells expressing MT1-MMP shows that, when compared with marimastat, significantly higher dithiol concentrations are required for active MT1-MMP binding and enhancement of pro-MMP-2 activation in the presence of TIMP-2.	bind
41407	4	9514	5	13	NULL	NULL	NULL	statement 3	Process		in the presence of					TIMP-2	GP				NULL	cells expressing MT1-MMP	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_13_11201_s_44	11790786	A comparative study of these compounds on the activation of pro-MMP-2 in cells expressing MT1-MMP shows that, when compared with marimastat, significantly higher dithiol concentrations are required for active MT1-MMP binding and enhancement of pro-MMP-2 activation in the presence of TIMP-2.	bind
41408	5	9514	5	13	NULL	NULL	NULL	dithiol	Chemical		is required for					MT1-MMP	GP	binding of active			NULL	cells expressing MT1-MMP	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_13_11201_s_44	11790786	A comparative study of these compounds on the activation of pro-MMP-2 in cells expressing MT1-MMP shows that, when compared with marimastat, significantly higher dithiol concentrations are required for active MT1-MMP binding and enhancement of pro-MMP-2 activation in the presence of TIMP-2.	bind
41409	6	9514	5	13	NULL	NULL	NULL	dithiol	Chemical		is required for					pro-MMP-2	GP	enhancement of;;activation of			NULL	cells expressing MT1-MMP	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_13_11201_s_44	11790786	A comparative study of these compounds on the activation of pro-MMP-2 in cells expressing MT1-MMP shows that, when compared with marimastat, significantly higher dithiol concentrations are required for active MT1-MMP binding and enhancement of pro-MMP-2 activation in the presence of TIMP-2.	bind
41410	7	9514	5	13	NULL	NULL	NULL	statement 6	Process		in the presence of					TIMP-2	GP				NULL	cells expressing MT1-MMP	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_13_11201_s_44	11790786	A comparative study of these compounds on the activation of pro-MMP-2 in cells expressing MT1-MMP shows that, when compared with marimastat, significantly higher dithiol concentrations are required for active MT1-MMP binding and enhancement of pro-MMP-2 activation in the presence of TIMP-2.	bind
40455	1	9514	7	10	NULL	0	NULL	MT1			bind					MMP					NULL	cells expressing MT1-MMP 	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_13_11201_s_44	11790786	A comparative study of these compounds on the activation of pro-MMP-2 in cells expressing MT1-MMP shows that, when compared with marimastat, significantly higher dithiol concentrations are required for active MT1-MMP binding and enhancement of pro-MMP-2 activation in the presence of TIMP-2.	bind
40457	2	9514	7	10	NULL	0	NULL	marimastat			is required for					statement 1		active			NULL	cells expressing MT1-MMP	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_13_11201_s_44	11790786	A comparative study of these compounds on the activation of pro-MMP-2 in cells expressing MT1-MMP shows that, when compared with marimastat, significantly higher dithiol concentrations are required for active MT1-MMP binding and enhancement of pro-MMP-2 activation in the presence of TIMP-2.	bind
40458	3	9514	7	10	NULL	0	NULL	dithiol 			is required for					statement 1		active			NULL	cells expressing MT1-MMP	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_13_11201_s_44	11790786	A comparative study of these compounds on the activation of pro-MMP-2 in cells expressing MT1-MMP shows that, when compared with marimastat, significantly higher dithiol concentrations are required for active MT1-MMP binding and enhancement of pro-MMP-2 activation in the presence of TIMP-2.	bind
40459	4	9514	7	10	NULL	0	NULL	 marimastat			is required for					pro-MMP-2		enhancement of;;activation of			NULL	cells expressing MT1-MMP	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_13_11201_s_44	11790786	A comparative study of these compounds on the activation of pro-MMP-2 in cells expressing MT1-MMP shows that, when compared with marimastat, significantly higher dithiol concentrations are required for active MT1-MMP binding and enhancement of pro-MMP-2 activation in the presence of TIMP-2.	bind
40460	5	9514	7	10	NULL	0	NULL	dithiol			is required for					pro-MMP-2		enhancement of;;activation of			NULL	cells expressing MT1-MMP	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_13_11201_s_44	11790786	A comparative study of these compounds on the activation of pro-MMP-2 in cells expressing MT1-MMP shows that, when compared with marimastat, significantly higher dithiol concentrations are required for active MT1-MMP binding and enhancement of pro-MMP-2 activation in the presence of TIMP-2.	bind
40461	6	9514	7	10	NULL	0	NULL	statement 4			in presence of					TIMP-2 					NULL	cells expressing MT1-MMP	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_13_11201_s_44	11790786	A comparative study of these compounds on the activation of pro-MMP-2 in cells expressing MT1-MMP shows that, when compared with marimastat, significantly higher dithiol concentrations are required for active MT1-MMP binding and enhancement of pro-MMP-2 activation in the presence of TIMP-2.	bind
40462	7	9514	7	10	NULL	0	NULL	statement 5			in presence of					TIMP-2 					NULL	cells expressing MT1-MMP	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_13_11201_s_44	11790786	A comparative study of these compounds on the activation of pro-MMP-2 in cells expressing MT1-MMP shows that, when compared with marimastat, significantly higher dithiol concentrations are required for active MT1-MMP binding and enhancement of pro-MMP-2 activation in the presence of TIMP-2.	bind
41411	1	9515	5	13	NULL	NULL	NULL	TPP+	GP		bind					EmrE	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_22_23_6175_s_72	14633977	A comparison between projection maps of native EmrE and TPP+-bound EmrE suggest only a minor conformational change between the two structures  (  et al).	bind
40463	1	9515	7	NULL	NULL	0	NULL	TPP+	NULL		bind	NULL				EmrE	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_22_23_6175_s_72	14633977	A comparison between projection maps of native EmrE and TPP+-bound EmrE suggest only a minor conformational change between the two structures  (  et al).	bind
41412	1	9516	5	13	NULL	NULL	NULL	FhuA	GP		is a type of					outer membrane receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_16_13966_s_169	11805094	A comparison between the binding modes of the outer membrane receptor FhuA and the periplasmic protein FhuD for albomycin is shown in Fig.  5.	bind
41413	2	9516	5	13	NULL	NULL	NULL	FhuA	GP		bind					albomycin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_16_13966_s_169	11805094	A comparison between the binding modes of the outer membrane receptor FhuA and the periplasmic protein FhuD for albomycin is shown in Fig.  5.	bind
41414	3	9516	5	13	NULL	NULL	NULL	FhuD	GP		is a type of					periplasmic protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_16_13966_s_169	11805094	A comparison between the binding modes of the outer membrane receptor FhuA and the periplasmic protein FhuD for albomycin is shown in Fig.  5.	bind
41415	4	9516	5	13	NULL	NULL	NULL	FhuD	GP		bind					albomycin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_16_13966_s_169	11805094	A comparison between the binding modes of the outer membrane receptor FhuA and the periplasmic protein FhuD for albomycin is shown in Fig.  5.	bind
40464	1	9516	7	NULL	NULL	0	NULL	FhuA	NULL		bind	NULL				albomycin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_16_13966_s_169	11805094	A comparison between the binding modes of the outer membrane receptor FhuA and the periplasmic protein FhuD for albomycin is shown in Fig.  5.	bind
40465	2	9516	7	NULL	NULL	0	NULL	FhuD	NULL		bind	NULL				albomycin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_16_13966_s_169	11805094	A comparison between the binding modes of the outer membrane receptor FhuA and the periplasmic protein FhuD for albomycin is shown in Fig.  5.	bind
40466	3	9516	7	NULL	NULL	0	NULL	FhuA	NULL		is a type of	NULL				outer membrane receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_16_13966_s_169	11805094	A comparison between the binding modes of the outer membrane receptor FhuA and the periplasmic protein FhuD for albomycin is shown in Fig.  5.	bind
40467	4	9516	7	NULL	NULL	0	NULL	FhuD	NULL		is a type of	NULL				 periplasmic protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_16_13966_s_169	11805094	A comparison between the binding modes of the outer membrane receptor FhuA and the periplasmic protein FhuD for albomycin is shown in Fig.  5.	bind
41416	1	9518	5	13	NULL	NULL	NULL	moesin	GP	WT	bind					GST-C-moesin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_18_12803_s_219	10212266	A comparison of  lanes 1 and  3 shows that PIP2 does not change binding between WT moesin and GST-C-moesin.	bind
41417	2	9518	5	13	NULL	NULL	NULL	PIP2	Chemical		does not change					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_18_12803_s_219	10212266	A comparison of  lanes 1 and  3 shows that PIP2 does not change binding between WT moesin and GST-C-moesin.	bind
40468	1	9518	7	NULL	NULL	0	NULL	WT moesin	NULL		bind	NULL				GST-C-moesin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_18_12803_s_219	10212266	A comparison of  lanes 1 and  3 shows that PIP2 does not change binding between WT moesin and GST-C-moesin.	bind
40469	2	9518	7	NULL	NULL	0	NULL	PIP2	NULL		does not change	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_18_12803_s_219	10212266	A comparison of  lanes 1 and  3 shows that PIP2 does not change binding between WT moesin and GST-C-moesin.	bind
42433	1	9519	5	13	NULL	NULL	NULL	126-base pair probe	NucleicAcid		is					alpha-Pal	GP			high affinity site	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34703_s_159	9856992	A comparison of alpha-Pal or Max, or both, binding activity using the 126-base pair probe shows that at low concentrations, neither factor alone can form stable complexes with the alpha-Pal high affinity site.	bind
42436	2	9519	5	13	NULL	NULL	NULL	alpha-Pal	GP		does not complex with					126-base pair probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34703_s_159	9856992	A comparison of alpha-Pal or Max, or both, binding activity using the 126-base pair probe shows that at low concentrations, neither factor alone can form stable complexes with the alpha-Pal high affinity site.	bind
42439	3	9519	5	13	NULL	NULL	NULL	Max	GP		does not complex with					126-base pair probe	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34703_s_159	9856992	A comparison of alpha-Pal or Max, or both, binding activity using the 126-base pair probe shows that at low concentrations, neither factor alone can form stable complexes with the alpha-Pal high affinity site.	bind
40471	1	9519	7	NULL	NULL	0	NULL	126-base pair probe	NULL		is	NULL				alpha-Pal	NULL			high affinity site	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34703_s_159	9856992	A comparison of alpha-Pal or Max, or both, binding activity using the 126-base pair probe shows that at low concentrations, neither factor alone can form stable complexes with the alpha-Pal high affinity site.	bind
40472	2	9519	7	NULL	NULL	0	NULL	alpha-Pal	NULL		does not complex with	NULL				126-base pair probe	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34703_s_159	9856992	A comparison of alpha-Pal or Max, or both, binding activity using the 126-base pair probe shows that at low concentrations, neither factor alone can form stable complexes with the alpha-Pal high affinity site.	bind
40757	3	9519	7	NULL	NULL	0	NULL	Max	NULL		does not complex with	NULL				126-base pair probe	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_52_34703_s_159	9856992	A comparison of alpha-Pal or Max, or both, binding activity using the 126-base pair probe shows that at low concentrations, neither factor alone can form stable complexes with the alpha-Pal high affinity site.	bind
41418	1	9520	5	13	NULL	NULL	NULL	Arf	GP		bind					GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1664_1_9_s_75	15238254	A comparison of Arf bound to GDP and to a nonhydrolyzable GTP analog revealed a unique  conformational switching mechanism in which GTP binding to Arf triggers the exposure  of the proteins' membrane anchor--a myristoylated amino-terminal  -helix ( Fig. 1B) [ 34].	bind
41419	2	9520	5	13	NULL	NULL	NULL	Arf	GP		bind					GTP analog	Chemical	nonhydrolyzable			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1664_1_9_s_75	15238254	A comparison of Arf bound to GDP and to a nonhydrolyzable GTP analog revealed a unique  conformational switching mechanism in which GTP binding to Arf triggers the exposure  of the proteins' membrane anchor--a myristoylated amino-terminal  -helix ( Fig. 1B) [ 34].	bind
41420	3	9520	5	13	NULL	NULL	NULL	GTP	Chemical		bind					Arf	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1664_1_9_s_75	15238254	A comparison of Arf bound to GDP and to a nonhydrolyzable GTP analog revealed a unique  conformational switching mechanism in which GTP binding to Arf triggers the exposure  of the proteins' membrane anchor--a myristoylated amino-terminal  -helix ( Fig. 1B) [ 34].	bind
41421	4	9520	5	13	NULL	NULL	NULL	myristoylated amino-terminal -helix	GP		is a type of 					proteins' membrane anchor	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1664_1_9_s_75	15238254	A comparison of Arf bound to GDP and to a nonhydrolyzable GTP analog revealed a unique  conformational switching mechanism in which GTP binding to Arf triggers the exposure  of the proteins' membrane anchor--a myristoylated amino-terminal  -helix ( Fig. 1B) [ 34].	bind
41422	5	9520	5	13	NULL	NULL	NULL	statement 3	Process		trigger					statement 4	GP	exposure of			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1664_1_9_s_75	15238254	A comparison of Arf bound to GDP and to a nonhydrolyzable GTP analog revealed a unique  conformational switching mechanism in which GTP binding to Arf triggers the exposure  of the proteins' membrane anchor--a myristoylated amino-terminal  -helix ( Fig. 1B) [ 34].	bind
40473	1	9520	7	NULL	NULL	0	NULL	Arf 	NULL		bind	NULL				GDP	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1664_1_9_s_75	15238254	A comparison of Arf bound to GDP and to a nonhydrolyzable GTP analog revealed a unique  conformational switching mechanism in which GTP binding to Arf triggers the exposure  of the proteins' membrane anchor--a myristoylated amino-terminal  -helix ( Fig. 1B) [ 34].	bind
40474	2	9520	7	NULL	NULL	0	NULL	Arf	NULL		bind	NULL				nonhydrolyzable GTP analog	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1664_1_9_s_75	15238254	A comparison of Arf bound to GDP and to a nonhydrolyzable GTP analog revealed a unique  conformational switching mechanism in which GTP binding to Arf triggers the exposure  of the proteins' membrane anchor--a myristoylated amino-terminal  -helix ( Fig. 1B) [ 34].	bind
40476	3	9520	7	NULL	NULL	0	NULL	Arf	NULL		bind	NULL				GTP	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1664_1_9_s_75	15238254	A comparison of Arf bound to GDP and to a nonhydrolyzable GTP analog revealed a unique  conformational switching mechanism in which GTP binding to Arf triggers the exposure  of the proteins' membrane anchor--a myristoylated amino-terminal  -helix ( Fig. 1B) [ 34].	bind
40479	4	9520	7	NULL	NULL	0	NULL	statement 3	NULL		triggers	NULL				myristoylated amino-terminal -helix 	NULL	exposure of			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1664_1_9_s_75	15238254	A comparison of Arf bound to GDP and to a nonhydrolyzable GTP analog revealed a unique  conformational switching mechanism in which GTP binding to Arf triggers the exposure  of the proteins' membrane anchor--a myristoylated amino-terminal  -helix ( Fig. 1B) [ 34].	bind
40480	5	9520	7	NULL	NULL	0	NULL	myristoylated amino-terminal -helix 	NULL		is a type of	NULL				proteins' membrane anchor	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1664_1_9_s_75	15238254	A comparison of Arf bound to GDP and to a nonhydrolyzable GTP analog revealed a unique  conformational switching mechanism in which GTP binding to Arf triggers the exposure  of the proteins' membrane anchor--a myristoylated amino-terminal  -helix ( Fig. 1B) [ 34].	bind
40483	6	9520	7	NULL	NULL	0	NULL	statement 1	NULL		compared with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1664_1_9_s_75	15238254	A comparison of Arf bound to GDP and to a nonhydrolyzable GTP analog revealed a unique  conformational switching mechanism in which GTP binding to Arf triggers the exposure  of the proteins' membrane anchor--a myristoylated amino-terminal  -helix ( Fig. 1B) [ 34].	bind
40484	7	9520	7	NULL	NULL	0	NULL	statement 6	NULL		reveals	NULL				unique conformational switching mechanism	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1664_1_9_s_75	15238254	A comparison of Arf bound to GDP and to a nonhydrolyzable GTP analog revealed a unique  conformational switching mechanism in which GTP binding to Arf triggers the exposure  of the proteins' membrane anchor--a myristoylated amino-terminal  -helix ( Fig. 1B) [ 34].	bind
41423	1	9521	5	13	NULL	NULL	NULL	GAD65	GP		interact with		distinctly			PLP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1645_1_63_s_232	12535612	A comparison of binding and formation constants between GAD65 and GAD67 reveals that  the two isoforms interact distinctly with the cofactor PLP.	bind
41424	2	9521	5	13	NULL	NULL	NULL	GAD67	GP		interact with		distinctly			PLP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1645_1_63_s_232	12535612	A comparison of binding and formation constants between GAD65 and GAD67 reveals that  the two isoforms interact distinctly with the cofactor PLP.	bind
41425	3	9521	5	13	NULL	NULL	NULL	PLP	Chemical		is a type of					cofactor	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1645_1_63_s_232	12535612	A comparison of binding and formation constants between GAD65 and GAD67 reveals that  the two isoforms interact distinctly with the cofactor PLP.	bind
40612	1	9521	7	NULL	NULL	0	NULL	GAD65	NULL		interacts with	NULL	distinctly			PLP	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1645_1_63_s_232	12535612	A comparison of binding and formation constants between GAD65 and GAD67 reveals that  the two isoforms interact distinctly with the cofactor PLP.	bind
40613	2	9521	7	NULL	NULL	0	NULL	GAD67	NULL		interacts with	NULL	distinctly			PLP	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1645_1_63_s_232	12535612	A comparison of binding and formation constants between GAD65 and GAD67 reveals that  the two isoforms interact distinctly with the cofactor PLP.	bind
56798	3	9521	7	10	NULL	0	NULL	PLP			is a type of					cofactor					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1645_1_63_s_232	12535612	A comparison of binding and formation constants between GAD65 and GAD67 reveals that  the two isoforms interact distinctly with the cofactor PLP.	bind
41427	1	9523	5	13	NULL	NULL	NULL	DDT	Chemical		bind					EcTS	GP				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_10_981_s_83	11590022	A comparison of DDT bound to EcTS to the antifolate ZD1694 bound to EcTS and hTS is shown in   Fig. 2 .	bind
41428	2	9523	5	13	NULL	NULL	NULL	ZD1694	Chemical		is a type of					antifolate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_10_981_s_83	11590022	A comparison of DDT bound to EcTS to the antifolate ZD1694 bound to EcTS and hTS is shown in   Fig. 2 .	bind
41429	3	9523	5	13	NULL	NULL	NULL	ZD1694	Chemical		bind					EcTS	GP				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_10_981_s_83	11590022	A comparison of DDT bound to EcTS to the antifolate ZD1694 bound to EcTS and hTS is shown in   Fig. 2 .	bind
41430	4	9523	5	13	NULL	NULL	NULL	ZD1694	Chemical		bind					hTS	GP				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_10_981_s_83	11590022	A comparison of DDT bound to EcTS to the antifolate ZD1694 bound to EcTS and hTS is shown in   Fig. 2 .	bind
40614	1	9523	7	NULL	NULL	0	NULL	DDT	NULL		bind	NULL				EcTS	NULL				NULL		0	NULL	NULL	NULL	gw60_chembiol_8_10_981_s_83	11590022	A comparison of DDT bound to EcTS to the antifolate ZD1694 bound to EcTS and hTS is shown in   Fig. 2 .	bind
40615	2	9523	7	10	NULL	0	NULL	ZD1694	NULL		bind	NULL				EcTS	NULL				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_10_981_s_83	11590022	A comparison of DDT bound to EcTS to the antifolate ZD1694 bound to EcTS and hTS is shown in   Fig. 2 .	bind
40616	3	9523	7	10	NULL	0	NULL	ZD1694	NULL		bind	NULL				hTS	NULL				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_10_981_s_83	11590022	A comparison of DDT bound to EcTS to the antifolate ZD1694 bound to EcTS and hTS is shown in   Fig. 2 .	bind
46865	4	9523	7	10	NULL	0	NULL	ZD1694	NULL		is a type of 	NULL				antifolate	NULL				NULL		0	NULL	NULL	NULL	gw60_chembiol_8_10_981_s_83	11590022	A comparison of DDT bound to EcTS to the antifolate ZD1694 bound to EcTS and hTS is shown in   Fig. 2 .	bind
41431	1	9524	5	13	NULL	NULL	NULL	flap endonuclease	GP		bind					pseudoY substrates	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_13_8542_s_9	12084915	A comparison of flap endonuclease binding to pseudoY substrates and duplexes with a single-stranded 5' overhang suggests a better model for 5' nuclease-DNA binding.	bind
41432	2	9524	5	13	NULL	NULL	NULL	flap endonuclease	GP		bind					duplexes	NucleicAcid			single-stranded 5' overhang	NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_13_8542_s_9	12084915	A comparison of flap endonuclease binding to pseudoY substrates and duplexes with a single-stranded 5' overhang suggests a better model for 5' nuclease-DNA binding.	bind
41433	3	9524	5	13	NULL	NULL	NULL	statement 1	Process		suggests					5' nuclease DNA	NucleicAcid	binding of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_13_8542_s_9	12084915	A comparison of flap endonuclease binding to pseudoY substrates and duplexes with a single-stranded 5' overhang suggests a better model for 5' nuclease-DNA binding.	bind
41434	4	9524	5	13	NULL	NULL	NULL	statement 1	Process		suggests					5' nuclease DNA	NucleicAcid	binding of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_13_8542_s_9	12084915	A comparison of flap endonuclease binding to pseudoY substrates and duplexes with a single-stranded 5' overhang suggests a better model for 5' nuclease-DNA binding.	bind
40617	1	9524	7	NULL	NULL	0	NULL	flap endonuclease	NULL		bind	NULL				pseudoY substrates	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_13_8542_s_9	12084915	A comparison of flap endonuclease binding to pseudoY substrates and duplexes with a single-stranded 5' overhang suggests a better model for 5' nuclease-DNA binding.	bind
40618	2	9524	7	NULL	NULL	0	NULL	flap endonuclease	NULL		bind	NULL				duplex	NULL			single-stranded 5' overhang	NULL		0	NULL	NULL	NULL	gw60_pnas_99_13_8542_s_9	12084915	A comparison of flap endonuclease binding to pseudoY substrates and duplexes with a single-stranded 5' overhang suggests a better model for 5' nuclease-DNA binding.	bind
40619	3	9524	7	NULL	NULL	0	NULL	statement 1	NULL		suggests	NULL				5'nuclease-DNA	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_pnas_99_13_8542_s_9	12084915	A comparison of flap endonuclease binding to pseudoY substrates and duplexes with a single-stranded 5' overhang suggests a better model for 5' nuclease-DNA binding.	bind
40620	4	9524	7	NULL	NULL	0	NULL	statement 2	NULL		suggests	NULL				5' nuclease-DNA	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_pnas_99_13_8542_s_9	12084915	A comparison of flap endonuclease binding to pseudoY substrates and duplexes with a single-stranded 5' overhang suggests a better model for 5' nuclease-DNA binding.	bind
41436	1	9525	5	13	NULL	NULL	NULL	Ugi	GP	[13C,15]	bind					Ung	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_34_21408_s_299	9261156	A comparison of free [15]Ugi (Fig.  9 A) to [13C,15]Ugi bound to Ung (Fig.  9 B) indicates that significant structural change of Ugi occurred as a consequence of complex formation.	bind
41437	2	9525	5	13	NULL	NULL	NULL	statement 1	Process		leads to					Ugi	GP	structural change of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_34_21408_s_299	9261156	A comparison of free [15]Ugi (Fig.  9 A) to [13C,15]Ugi bound to Ung (Fig.  9 B) indicates that significant structural change of Ugi occurred as a consequence of complex formation.	bind
56799	3	9525	5	13	NULL	NULL	NULL	Ugi	GP	free	bind					Ung	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_34_21408_s_299	9261156	A comparison of free [15]Ugi (Fig.  9 A) to [13C,15]Ugi bound to Ung (Fig.  9 B) indicates that significant structural change of Ugi occurred as a consequence of complex formation.	bind
40621	1	9525	7	10	NULL	0	NULL	Ugi	NULL	free	bind	NULL				Ung	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_34_21408_s_299	9261156	A comparison of free [15]Ugi (Fig.  9 A) to [13C,15]Ugi bound to Ung (Fig.  9 B) indicates that significant structural change of Ugi occurred as a consequence of complex formation.	bind
40622	2	9525	7	10	NULL	0	NULL	Ugi 	NULL	[13C,15]	bind	NULL				Ung	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_34_21408_s_299	9261156	A comparison of free [15]Ugi (Fig.  9 A) to [13C,15]Ugi bound to Ung (Fig.  9 B) indicates that significant structural change of Ugi occurred as a consequence of complex formation.	bind
40623	3	9525	7	10	NULL	0	NULL	statement 1			leads to					Ugi		structural change of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_34_21408_s_299	9261156	A comparison of free [15]Ugi (Fig.  9 A) to [13C,15]Ugi bound to Ung (Fig.  9 B) indicates that significant structural change of Ugi occurred as a consequence of complex formation.	bind
41438	1	9526	5	13	NULL	NULL	NULL	GST-FinO	GP		bind					FinP	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_15_10356_s_74	10187824	A comparison of GST-FinO binding affinities to FinP, SLI (nucleotides 1-34, Fig.  1) and SLII (nucleotides 35-79), which were transcribed from PCR-generated templates, is shown in Fig.  3.	bind
41439	2	9526	5	13	NULL	NULL	NULL	GST-FinO	GP		bind					SLI	NucleicAcid			nucleotides 1-34	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_15_10356_s_74	10187824	A comparison of GST-FinO binding affinities to FinP, SLI (nucleotides 1-34, Fig.  1) and SLII (nucleotides 35-79), which were transcribed from PCR-generated templates, is shown in Fig.  3.	bind
41440	3	9526	5	13	NULL	NULL	NULL	GST-FinO	GP		bind					SLII	NucleicAcid			nucleotides 35-79	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_15_10356_s_74	10187824	A comparison of GST-FinO binding affinities to FinP, SLI (nucleotides 1-34, Fig.  1) and SLII (nucleotides 35-79), which were transcribed from PCR-generated templates, is shown in Fig.  3.	bind
40625	1	9526	7	NULL	NULL	0	NULL	GST-FinO	NULL		bind	NULL				FinP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_15_10356_s_74	10187824	A comparison of GST-FinO binding affinities to FinP, SLI (nucleotides 1-34, Fig.  1) and SLII (nucleotides 35-79), which were transcribed from PCR-generated templates, is shown in Fig.  3.	bind
40626	2	9526	7	NULL	NULL	0	NULL	GST-FinO	NULL		bind	NULL				SL1	NULL			nucleotides 1-34	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_15_10356_s_74	10187824	A comparison of GST-FinO binding affinities to FinP, SLI (nucleotides 1-34, Fig.  1) and SLII (nucleotides 35-79), which were transcribed from PCR-generated templates, is shown in Fig.  3.	bind
40627	3	9526	7	NULL	NULL	0	NULL	GST-FinO	NULL		bind	NULL				SLII	NULL			nucleotides 35-79	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_15_10356_s_74	10187824	A comparison of GST-FinO binding affinities to FinP, SLI (nucleotides 1-34, Fig.  1) and SLII (nucleotides 35-79), which were transcribed from PCR-generated templates, is shown in Fig.  3.	bind
41441	1	9527	5	13	NULL	NULL	NULL	HIV-1 RT	GP		bind		effectively			ATP	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_plos-pathog_2_2_16485036_s_10	16485036	A comparison of HIV-1 and  HIV-2 RT shows that there are numerous differences in the putative ATP  binding sites that could explain why HIV-1 RT binds ATP more effectively.	bind
40628	1	9527	7	NULL	NULL	0	NULL	 HIV-1 RT	NULL		binds	NULL	effectively			ATP	NULL				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_plos-pathog_2_2_16485036_s_10	16485036	A comparison of HIV-1 and  HIV-2 RT shows that there are numerous differences in the putative ATP  binding sites that could explain why HIV-1 RT binds ATP more effectively.	bind
41442	1	9528	5	13	NULL	NULL	NULL	hMSH2	GP		bind					hMSH6	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_36_27851_s_79	10878012	A comparison of hMSH2-hMSH6 binding affinity suggests G/T   +CA > mG/T > mG/C   G/C.	bind
42417	2	9528	5	NULL	NULL	0	NULL		NULL	binding affinity of	greater than	NULL			G/T +CA		NULL	binding affinity of		mG/T	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_36_27851_s_79	10878012	A comparison of hMSH2-hMSH6 binding affinity suggests G/T   +CA > mG/T > mG/C   G/C.	bind
42418	3	9528	5	13	NULL	NULL	NULL	statement 2	Process	binding affinity of	greater than							binding affinity of		mG/C	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_36_27851_s_79	10878012	A comparison of hMSH2-hMSH6 binding affinity suggests G/T   +CA > mG/T > mG/C   G/C.	bind
40630	1	9528	7	NULL	NULL	0	NULL	hMSH2	NULL		bind	NULL				hMSH6	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_36_27851_s_79	10878012	A comparison of hMSH2-hMSH6 binding affinity suggests G/T   +CA > mG/T > mG/C   G/C.	bind
40631	2	9528	7	10	NULL	0	NULL			binding affinity of	is greater than				G/T +CA			binding affinity of		 mG/T	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_36_27851_s_79	10878012	A comparison of hMSH2-hMSH6 binding affinity suggests G/T   +CA > mG/T > mG/C   G/C.	bind
40632	3	9528	7	10	NULL	0	NULL	statement 2		binding affinity of	is greater than							binding affinity of		mG/C G/C	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_36_27851_s_79	10878012	A comparison of hMSH2-hMSH6 binding affinity suggests G/T   +CA > mG/T > mG/C   G/C.	bind
41443	1	9529	5	13	NULL	NULL	NULL	MARCKS	GP		bind			PSD		G-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_25_22351_s_162	11294839	A Comparison of MARCKS PSD Binding to F- and G-actin Reveals Localizing Interactions between MARCKS and F-actin-- Binding of the N-terminal PSD peptide to F-actin is increased relative to G-actin by a factor of less than 2 (Fig.  5 A,  inset).	bind
41444	2	9529	5	13	NULL	NULL	NULL	MARCKS	GP		bind			PSD		F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_25_22351_s_162	11294839	A Comparison of MARCKS PSD Binding to F- and G-actin Reveals Localizing Interactions between MARCKS and F-actin-- Binding of the N-terminal PSD peptide to F-actin is increased relative to G-actin by a factor of less than 2 (Fig.  5 A,  inset).	bind
41445	3	9529	5	13	NULL	NULL	NULL	PSD peptide	GP		bind			N-terminal		F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_25_22351_s_162	11294839	A Comparison of MARCKS PSD Binding to F- and G-actin Reveals Localizing Interactions between MARCKS and F-actin-- Binding of the N-terminal PSD peptide to F-actin is increased relative to G-actin by a factor of less than 2 (Fig.  5 A,  inset).	bind
41446	4	9529	5	13	NULL	NULL	NULL	PSD peptide	GP		bind			N-terminal		G-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_25_22351_s_162	11294839	A Comparison of MARCKS PSD Binding to F- and G-actin Reveals Localizing Interactions between MARCKS and F-actin-- Binding of the N-terminal PSD peptide to F-actin is increased relative to G-actin by a factor of less than 2 (Fig.  5 A,  inset).	bind
41447	5	9529	5	13	NULL	NULL	NULL	statement 3	Process		is relative to		increased			statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_25_22351_s_162	11294839	A Comparison of MARCKS PSD Binding to F- and G-actin Reveals Localizing Interactions between MARCKS and F-actin-- Binding of the N-terminal PSD peptide to F-actin is increased relative to G-actin by a factor of less than 2 (Fig.  5 A,  inset).	bind
40635	1	9529	7	10	NULL	0	NULL	MARCKS 	NULL		bind	NULL		PSD		F-actin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_25_22351_s_162	11294839	A Comparison of MARCKS PSD Binding to F- and G-actin Reveals Localizing Interactions between MARCKS and F-actin-- Binding of the N-terminal PSD peptide to F-actin is increased relative to G-actin by a factor of less than 2 (Fig.  5 A,  inset).	bind
40636	2	9529	7	10	NULL	0	NULL	MARCKS	NULL		bind	NULL		PSD		G-actin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_25_22351_s_162	11294839	A Comparison of MARCKS PSD Binding to F- and G-actin Reveals Localizing Interactions between MARCKS and F-actin-- Binding of the N-terminal PSD peptide to F-actin is increased relative to G-actin by a factor of less than 2 (Fig.  5 A,  inset).	bind
40637	3	9529	7	NULL	NULL	0	NULL	PSD peptide	NULL		bind	NULL		N-terminal		F-actin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_25_22351_s_162	11294839	A Comparison of MARCKS PSD Binding to F- and G-actin Reveals Localizing Interactions between MARCKS and F-actin-- Binding of the N-terminal PSD peptide to F-actin is increased relative to G-actin by a factor of less than 2 (Fig.  5 A,  inset).	bind
40638	4	9529	7	NULL	NULL	0	NULL	PSD peptide	NULL		bind	NULL		N-terminal 		G-actin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_25_22351_s_162	11294839	A Comparison of MARCKS PSD Binding to F- and G-actin Reveals Localizing Interactions between MARCKS and F-actin-- Binding of the N-terminal PSD peptide to F-actin is increased relative to G-actin by a factor of less than 2 (Fig.  5 A,  inset).	bind
40639	5	9529	7	NULL	NULL	0	NULL	statement 3	NULL	binding of	is increased than	NULL				statement 4	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_25_22351_s_162	11294839	A Comparison of MARCKS PSD Binding to F- and G-actin Reveals Localizing Interactions between MARCKS and F-actin-- Binding of the N-terminal PSD peptide to F-actin is increased relative to G-actin by a factor of less than 2 (Fig.  5 A,  inset).	bind
41448	1	9530	5	13	NULL	NULL	NULL	p42Ets-1	GP		bind					DNA sequences	NucleicAcid				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_oncogene_22_57_14668797_s_5	14668797	A comparison of optimal DNA-binding sites shows that  p42Ets-1 binds to more various DNA sequences than p51Ets-1; p42Ets-1 recognizes  the same optimal consensus sequence as p51Ets-1, but also many variations  of it, mainly at base -1, which is located just prior to the GGAA/T core  sequence.	bind
41449	2	9530	5	13	NULL	NULL	NULL	p51Ets-1	GP		bind					DNA sequences	NucleicAcid				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_oncogene_22_57_14668797_s_5	14668797	A comparison of optimal DNA-binding sites shows that  p42Ets-1 binds to more various DNA sequences than p51Ets-1; p42Ets-1 recognizes  the same optimal consensus sequence as p51Ets-1, but also many variations  of it, mainly at base -1, which is located just prior to the GGAA/T core  sequence.	bind
40640	1	9530	7	10	NULL	0	NULL	p42Ets-1			binds to					consensus DNA sequence				 	NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_oncogene_22_57_14668797_s_5	14668797	A comparison of optimal DNA-binding sites shows that  p42Ets-1 binds to more various DNA sequences than p51Ets-1; p42Ets-1 recognizes  the same optimal consensus sequence as p51Ets-1, but also many variations  of it, mainly at base -1, which is located just prior to the GGAA/T core  sequence.	bind
40641	2	9530	7	10	NULL	0	NULL	p51Ets-1			bind					consensus DNA sequence					NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_oncogene_22_57_14668797_s_5	14668797	A comparison of optimal DNA-binding sites shows that  p42Ets-1 binds to more various DNA sequences than p51Ets-1; p42Ets-1 recognizes  the same optimal consensus sequence as p51Ets-1, but also many variations  of it, mainly at base -1, which is located just prior to the GGAA/T core  sequence.	bind
41731	1	9531	5	13	NULL	NULL	NULL	Hsp90	GP		bind			Lys-40		PP5	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_43_40799_s_242	12145316	A comparison of our CyP40 mutational analysis data (Fig.  4) with that for PP5 ( 29) demonstrated complete concordance with the relative extent of Hsp90 binding to PP5, in that the status of nonbinding residues Lys-32, Lys-97, and Arg-101 (CyP40 residues Lys-227, Lys-308, and Arg-312, respectively), partial binders Arg-74 and Ile-63 (CyP40 residues Lys-285 and Ser-274, respectively), and the full binder Lys-40 (CyP40 residue Lys-235) was the same.	bind
42427	2	9531	5	13	NULL	NULL	NULL	PP5	GP		is not involved in			Lys-32		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_43_40799_s_242	12145316	A comparison of our CyP40 mutational analysis data (Fig.  4) with that for PP5 ( 29) demonstrated complete concordance with the relative extent of Hsp90 binding to PP5, in that the status of nonbinding residues Lys-32, Lys-97, and Arg-101 (CyP40 residues Lys-227, Lys-308, and Arg-312, respectively), partial binders Arg-74 and Ile-63 (CyP40 residues Lys-285 and Ser-274, respectively), and the full binder Lys-40 (CyP40 residue Lys-235) was the same.	bind
42428	3	9531	5	13	NULL	NULL	NULL	PP5	GP		is not involved in			Lys-97		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_43_40799_s_242	12145316	A comparison of our CyP40 mutational analysis data (Fig.  4) with that for PP5 ( 29) demonstrated complete concordance with the relative extent of Hsp90 binding to PP5, in that the status of nonbinding residues Lys-32, Lys-97, and Arg-101 (CyP40 residues Lys-227, Lys-308, and Arg-312, respectively), partial binders Arg-74 and Ile-63 (CyP40 residues Lys-285 and Ser-274, respectively), and the full binder Lys-40 (CyP40 residue Lys-235) was the same.	bind
42429	4	9531	5	13	NULL	NULL	NULL	PP5	GP		is not involved in			Arg-101		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_43_40799_s_242	12145316	A comparison of our CyP40 mutational analysis data (Fig.  4) with that for PP5 ( 29) demonstrated complete concordance with the relative extent of Hsp90 binding to PP5, in that the status of nonbinding residues Lys-32, Lys-97, and Arg-101 (CyP40 residues Lys-227, Lys-308, and Arg-312, respectively), partial binders Arg-74 and Ile-63 (CyP40 residues Lys-285 and Ser-274, respectively), and the full binder Lys-40 (CyP40 residue Lys-235) was the same.	bind
42430	5	9531	5	13	NULL	NULL	NULL	PP5	GP		is involved in		partially	Arg-74		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_43_40799_s_242	12145316	A comparison of our CyP40 mutational analysis data (Fig.  4) with that for PP5 ( 29) demonstrated complete concordance with the relative extent of Hsp90 binding to PP5, in that the status of nonbinding residues Lys-32, Lys-97, and Arg-101 (CyP40 residues Lys-227, Lys-308, and Arg-312, respectively), partial binders Arg-74 and Ile-63 (CyP40 residues Lys-285 and Ser-274, respectively), and the full binder Lys-40 (CyP40 residue Lys-235) was the same.	bind
42431	6	9531	5	13	NULL	NULL	NULL	PP5	GP		is involved in		partially	Ile-63		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_43_40799_s_242	12145316	A comparison of our CyP40 mutational analysis data (Fig.  4) with that for PP5 ( 29) demonstrated complete concordance with the relative extent of Hsp90 binding to PP5, in that the status of nonbinding residues Lys-32, Lys-97, and Arg-101 (CyP40 residues Lys-227, Lys-308, and Arg-312, respectively), partial binders Arg-74 and Ile-63 (CyP40 residues Lys-285 and Ser-274, respectively), and the full binder Lys-40 (CyP40 residue Lys-235) was the same.	bind
40643	1	9531	7	NULL	NULL	0	NULL	Hsp90	NULL		bind	NULL		Lys-40		PP5	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_43_40799_s_242	12145316	A comparison of our CyP40 mutational analysis data (Fig.  4) with that for PP5 ( 29) demonstrated complete concordance with the relative extent of Hsp90 binding to PP5, in that the status of nonbinding residues Lys-32, Lys-97, and Arg-101 (CyP40 residues Lys-227, Lys-308, and Arg-312, respectively), partial binders Arg-74 and Ile-63 (CyP40 residues Lys-285 and Ser-274, respectively), and the full binder Lys-40 (CyP40 residue Lys-235) was the same.	bind
40644	2	9531	7	NULL	NULL	0	NULL	PP5	NULL		is not involved in	NULL		Lys-32		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_43_40799_s_242	12145316	A comparison of our CyP40 mutational analysis data (Fig.  4) with that for PP5 ( 29) demonstrated complete concordance with the relative extent of Hsp90 binding to PP5, in that the status of nonbinding residues Lys-32, Lys-97, and Arg-101 (CyP40 residues Lys-227, Lys-308, and Arg-312, respectively), partial binders Arg-74 and Ile-63 (CyP40 residues Lys-285 and Ser-274, respectively), and the full binder Lys-40 (CyP40 residue Lys-235) was the same.	bind
40645	3	9531	7	NULL	NULL	0	NULL	PP5	NULL		is not involved in	NULL		Lys-97		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_43_40799_s_242	12145316	A comparison of our CyP40 mutational analysis data (Fig.  4) with that for PP5 ( 29) demonstrated complete concordance with the relative extent of Hsp90 binding to PP5, in that the status of nonbinding residues Lys-32, Lys-97, and Arg-101 (CyP40 residues Lys-227, Lys-308, and Arg-312, respectively), partial binders Arg-74 and Ile-63 (CyP40 residues Lys-285 and Ser-274, respectively), and the full binder Lys-40 (CyP40 residue Lys-235) was the same.	bind
40646	4	9531	7	NULL	NULL	0	NULL	PP5	NULL		is not involved in	NULL		 Arg-101		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_43_40799_s_242	12145316	A comparison of our CyP40 mutational analysis data (Fig.  4) with that for PP5 ( 29) demonstrated complete concordance with the relative extent of Hsp90 binding to PP5, in that the status of nonbinding residues Lys-32, Lys-97, and Arg-101 (CyP40 residues Lys-227, Lys-308, and Arg-312, respectively), partial binders Arg-74 and Ile-63 (CyP40 residues Lys-285 and Ser-274, respectively), and the full binder Lys-40 (CyP40 residue Lys-235) was the same.	bind
40647	5	9531	7	NULL	NULL	0	NULL	PP5	NULL		is involved in	NULL	partially	Arg-74		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_43_40799_s_242	12145316	A comparison of our CyP40 mutational analysis data (Fig.  4) with that for PP5 ( 29) demonstrated complete concordance with the relative extent of Hsp90 binding to PP5, in that the status of nonbinding residues Lys-32, Lys-97, and Arg-101 (CyP40 residues Lys-227, Lys-308, and Arg-312, respectively), partial binders Arg-74 and Ile-63 (CyP40 residues Lys-285 and Ser-274, respectively), and the full binder Lys-40 (CyP40 residue Lys-235) was the same.	bind
40648	6	9531	7	NULL	NULL	0	NULL	PP5	NULL		is involved in	NULL	partially	Ile-63		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_43_40799_s_242	12145316	A comparison of our CyP40 mutational analysis data (Fig.  4) with that for PP5 ( 29) demonstrated complete concordance with the relative extent of Hsp90 binding to PP5, in that the status of nonbinding residues Lys-32, Lys-97, and Arg-101 (CyP40 residues Lys-227, Lys-308, and Arg-312, respectively), partial binders Arg-74 and Ile-63 (CyP40 residues Lys-285 and Ser-274, respectively), and the full binder Lys-40 (CyP40 residue Lys-235) was the same.	bind
41453	1	9532	5	13	NULL	NULL	NULL	p47	GP		bind			C terminus		p97	GP		ND1		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_5_1030_s_68	14988733	A comparison of p47 C bound to p97 ND1 with the solution structure of p47 UBX ( Figure 2A,  Table II) shows differences in the N-terminal part, which may be due to the shorter fragment  used for the solution structure determination (282 370).	bind
40649	1	9532	7	10	NULL	0	NULL	 p47	NULL		binds to	NULL		 C terminus		p97 	NULL		ND1		NULL		NULL	NULL	NULL	NULL	gw70_embo_23_5_1030_s_68	14988733	A comparison of p47 C bound to p97 ND1 with the solution structure of p47 UBX ( Figure 2A,  Table II) shows differences in the N-terminal part, which may be due to the shorter fragment  used for the solution structure determination (282 370).	bind
41454	1	9533	5	13	NULL	NULL	NULL	R1	GP		bind					AMA1	GP	recombinant;;P. falciparum			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_10_6981_s_151	16177378	A comparison of R1 binding to recombinant AMA1 from four different lines of  P. falciparum demonstrated that R1 recognizes AMA1 from the D10 line of  P. falciparum, as well as 3D7  PfAMA1, the form of the antigen used for panning.	bind
41455	2	9533	5	13	NULL	NULL	NULL	R1	GP		recognizes					AMA1	GP	D10 line of P. falciparum			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_10_6981_s_151	16177378	A comparison of R1 binding to recombinant AMA1 from four different lines of  P. falciparum demonstrated that R1 recognizes AMA1 from the D10 line of  P. falciparum, as well as 3D7  PfAMA1, the form of the antigen used for panning.	bind
41456	3	9533	5	13	NULL	NULL	NULL	R1	GP		recognizes					AMA1	GP	3D7;; P. falciparum			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_10_6981_s_151	16177378	A comparison of R1 binding to recombinant AMA1 from four different lines of  P. falciparum demonstrated that R1 recognizes AMA1 from the D10 line of  P. falciparum, as well as 3D7  PfAMA1, the form of the antigen used for panning.	bind
40650	1	9533	7	10	NULL	0	NULL	R1	NULL		bind	NULL				AMA1	NULL	recombinant;; P. falciparum			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_10_6981_s_151	16177378	A comparison of R1 binding to recombinant AMA1 from four different lines of  P. falciparum demonstrated that R1 recognizes AMA1 from the D10 line of  P. falciparum, as well as 3D7  PfAMA1, the form of the antigen used for panning.	bind
40651	2	9533	7	10	NULL	0	NULL	R1	NULL		recognizes	NULL				AMA1	NULL	D10 line of P. falciparum			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_10_6981_s_151	16177378	A comparison of R1 binding to recombinant AMA1 from four different lines of  P. falciparum demonstrated that R1 recognizes AMA1 from the D10 line of  P. falciparum, as well as 3D7  PfAMA1, the form of the antigen used for panning.	bind
40652	3	9533	7	10	NULL	0	NULL	R1	NULL		recognizes	NULL				AMA1	NULL	3D7;; P. falciparum			NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_73_10_6981_s_151	16177378	A comparison of R1 binding to recombinant AMA1 from four different lines of  P. falciparum demonstrated that R1 recognizes AMA1 from the D10 line of  P. falciparum, as well as 3D7  PfAMA1, the form of the antigen used for panning.	bind
41459	1	9534	5	13	NULL	NULL	NULL	SAP	GP		bind					laminin	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2143_s_118	8999915	A comparison of SAP binding to human and mouse laminin indicates that SAP binding to human laminin is lower than SAP binding to mouse laminin (Fig.  3 A).	bind
41460	2	9534	5	13	NULL	NULL	NULL	SAP	GP		bind					laminin	GP	mouse			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2143_s_118	8999915	A comparison of SAP binding to human and mouse laminin indicates that SAP binding to human laminin is lower than SAP binding to mouse laminin (Fig.  3 A).	bind
41461	3	9534	5	13	NULL	NULL	NULL	statement 1	Process		lower than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2143_s_118	8999915	A comparison of SAP binding to human and mouse laminin indicates that SAP binding to human laminin is lower than SAP binding to mouse laminin (Fig.  3 A).	bind
40653	1	9534	7	NULL	NULL	0	NULL	SAP	NULL		bind	NULL				laminin	NULL	human			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_4_2143_s_118	8999915	A comparison of SAP binding to human and mouse laminin indicates that SAP binding to human laminin is lower than SAP binding to mouse laminin (Fig.  3 A).	bind
40654	2	9534	7	NULL	NULL	0	NULL	SAP	NULL		bind	NULL				laminin	NULL	mouse			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_4_2143_s_118	8999915	A comparison of SAP binding to human and mouse laminin indicates that SAP binding to human laminin is lower than SAP binding to mouse laminin (Fig.  3 A).	bind
40655	3	9534	7	NULL	NULL	0	NULL	statement 1	NULL	binding of	is lower than	NULL				statement 2	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_4_2143_s_118	8999915	A comparison of SAP binding to human and mouse laminin indicates that SAP binding to human laminin is lower than SAP binding to mouse laminin (Fig.  3 A).	bind
41462	1	9535	5	13	NULL	NULL	NULL	SHC	GP		bind			PTB domain		substrates	GP	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_9_1134_s_41	8805372	A comparison of SHC and NUMB PTB domains shows that amino acids critical for the binding of the SHC PTB domain to tyrosine-phosphorylated substrates are conserved in the mNUMB protein    [24-26]   (  Figure 1c).	bind
41463	2	9535	5	13	NULL	NULL	NULL	SHC	GP		is conserved in			amino acid PTB domain		mNUMB protein	GP		amino acid PTB domain		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_9_1134_s_41	8805372	A comparison of SHC and NUMB PTB domains shows that amino acids critical for the binding of the SHC PTB domain to tyrosine-phosphorylated substrates are conserved in the mNUMB protein    [24-26]   (  Figure 1c).	bind
56903	3	9535	5	13	NULL	NULL	NULL	mNUMB protein	GP		bind			PTB domain		substrates	GP	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_9_1134_s_41	8805372	A comparison of SHC and NUMB PTB domains shows that amino acids critical for the binding of the SHC PTB domain to tyrosine-phosphorylated substrates are conserved in the mNUMB protein    [24-26]   (  Figure 1c).	bind
40656	1	9535	7	NULL	NULL	0	NULL	SHC	NULL		bind	NULL		PTB domain		substrates	NULL	phosphorylated	tyrosine		NULL		0	NULL	NULL	NULL	gw60_currbiol_6_9_1134_s_41	8805372	A comparison of SHC and NUMB PTB domains shows that amino acids critical for the binding of the SHC PTB domain to tyrosine-phosphorylated substrates are conserved in the mNUMB protein    [24-26]   (  Figure 1c).	bind
40657	2	9535	7	NULL	NULL	0	NULL	mNUMB protein	NULL		bind	NULL		PTB domain		substrates	NULL	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_9_1134_s_41	8805372	A comparison of SHC and NUMB PTB domains shows that amino acids critical for the binding of the SHC PTB domain to tyrosine-phosphorylated substrates are conserved in the mNUMB protein    [24-26]   (  Figure 1c).	bind
40658	3	9535	7	NULL	NULL	0	NULL	SHC	NULL		is conserved in	NULL		aminoacid PTB domain		mNUMB protein	NULL		aminoacid PTB domain		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_9_1134_s_41	8805372	A comparison of SHC and NUMB PTB domains shows that amino acids critical for the binding of the SHC PTB domain to tyrosine-phosphorylated substrates are conserved in the mNUMB protein    [24-26]   (  Figure 1c).	bind
41464	1	9536	5	13	NULL	NULL	NULL	T1E	GP		bind					ErbB1	GP		Domain I		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_40_39114_s_169	12869572	A Comparison of T1E Binding to ErbB1 Domain I and ErbB3 Domain I -- T1E is unique in its properties since it can bind both to ErbB1 and ErbB3.	bind
41465	2	9536	5	13	NULL	NULL	NULL	T1E	GP		bind					ErbB3	GP		Domain I		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_40_39114_s_169	12869572	A Comparison of T1E Binding to ErbB1 Domain I and ErbB3 Domain I -- T1E is unique in its properties since it can bind both to ErbB1 and ErbB3.	bind
40659	1	9536	7	NULL	NULL	0	NULL	 T1E	NULL		bind	NULL				 ErbB1	NULL		Domain I		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_40_39114_s_169	12869572	A Comparison of T1E Binding to ErbB1 Domain I and ErbB3 Domain I -- T1E is unique in its properties since it can bind both to ErbB1 and ErbB3.	bind
40660	2	9536	7	NULL	NULL	0	NULL	T1E	NULL		bind	NULL				ErbB3	NULL		Domain I		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_40_39114_s_169	12869572	A Comparison of T1E Binding to ErbB1 Domain I and ErbB3 Domain I -- T1E is unique in its properties since it can bind both to ErbB1 and ErbB3.	bind
41466	1	9537	5	13	NULL	NULL	NULL	holo-Tf	GP		bind					TfR1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_22_16618_s_203	10748106	A comparison of Tf binding to TfR1 and TfR2-alpha cells found that the affinity of holo-Tf for TfR2-alpha was substantially lower than for TfR1.	bind
41467	2	9537	5	13	NULL	NULL	NULL	holo-Tf	GP		bind					TfR2-alpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_22_16618_s_203	10748106	A comparison of Tf binding to TfR1 and TfR2-alpha cells found that the affinity of holo-Tf for TfR2-alpha was substantially lower than for TfR1.	bind
41468	3	9537	5	13	NULL	NULL	NULL	statement 2	Process		lower than		substantially			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_22_16618_s_203	10748106	A comparison of Tf binding to TfR1 and TfR2-alpha cells found that the affinity of holo-Tf for TfR2-alpha was substantially lower than for TfR1.	bind
40661	1	9537	7	10	NULL	0	NULL	holo-Tf			bind					TfR1-alpha cells					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_22_16618_s_203	10748106	A comparison of Tf binding to TfR1 and TfR2-alpha cells found that the affinity of holo-Tf for TfR2-alpha was substantially lower than for TfR1.	bind
40662	2	9537	7	10	NULL	0	NULL	holo-Tf			bind					TfR2-alpha cells					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_22_16618_s_203	10748106	A comparison of Tf binding to TfR1 and TfR2-alpha cells found that the affinity of holo-Tf for TfR2-alpha was substantially lower than for TfR1.	bind
40664	3	9537	7	10	NULL	0	NULL	statement 2		affinity of 	is lower than		substantially			statement 3		affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_22_16618_s_203	10748106	A comparison of Tf binding to TfR1 and TfR2-alpha cells found that the affinity of holo-Tf for TfR2-alpha was substantially lower than for TfR1.	bind
41469	1	9538	5	13	NULL	NULL	NULL	ASA-BZ-photolabeled peptides 	GP	H. contortus	bind		weakly	N-terminal 63-103		tubulin	GP	mammalian			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_15_8575_s_247	8621485	A comparison of the  amino acid sequence of ASA-BZ-photolabeled peptides (N-terminal  63-103) of  H. contortus  to bovine or human beta-tubulin  show two different amino acid residues (Ala    Gln and  Leu    Ile) that could confer weaker binding of BZ to  mammalian tubulin.	bind
40665	1	9538	7	10	NULL	0	NULL	ASA-BZ-photolabeled peptides 		H. contortus	bind		weakly	N-terminal 63-103		tubulin		mammalian			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_15_8575_s_247	8621485	A comparison of the  amino acid sequence of ASA-BZ-photolabeled peptides (N-terminal  63-103) of  H. contortus  to bovine or human beta-tubulin  show two different amino acid residues (Ala    Gln and  Leu    Ile) that could confer weaker binding of BZ to  mammalian tubulin.	bind
41470	1	9539	5	13	NULL	NULL	NULL	scFv	GP	bivalent	bind					BSA-A-trisaccharide	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2059_s_144	11679577	A comparison of the  K D values for bivalent scFv binding with BSA-A-trisaccharide  versus monovalent trisaccharide binding to scFv indicated that the avidity gain afforded by bivalency was ~75-fold for the L(103H)I and L(103H)V mutants.	bind
41471	2	9539	5	13	NULL	NULL	NULL	trisaccharide	Chemical	monovalent	bind					scFv	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2059_s_144	11679577	A comparison of the  K D values for bivalent scFv binding with BSA-A-trisaccharide  versus monovalent trisaccharide binding to scFv indicated that the avidity gain afforded by bivalency was ~75-fold for the L(103H)I and L(103H)V mutants.	bind
41704	3	9539	5	13	NULL	NULL	NULL	scFv	GP	bivalent;;mutant	increase			L(103H)I		statement 1	Process	avidity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2059_s_144	11679577	A comparison of the  K D values for bivalent scFv binding with BSA-A-trisaccharide  versus monovalent trisaccharide binding to scFv indicated that the avidity gain afforded by bivalency was ~75-fold for the L(103H)I and L(103H)V mutants.	bind
41705	4	9539	5	13	NULL	NULL	NULL	scFv	GP	bivalent;;mutant	increase			L(103H)V		statement 1	Process	avidity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2059_s_144	11679577	A comparison of the  K D values for bivalent scFv binding with BSA-A-trisaccharide  versus monovalent trisaccharide binding to scFv indicated that the avidity gain afforded by bivalency was ~75-fold for the L(103H)I and L(103H)V mutants.	bind
40670	1	9539	7	10	NULL	0	NULL	scFv		bivalent 	bind					BSA-A-trisaccharide					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2059_s_144	11679577	A comparison of the  K D values for bivalent scFv binding with BSA-A-trisaccharide  versus monovalent trisaccharide binding to scFv indicated that the avidity gain afforded by bivalency was ~75-fold for the L(103H)I and L(103H)V mutants.	bind
40671	2	9539	7	10	NULL	0	NULL	scFv			bind					 trisaccharide		monovalent			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2059_s_144	11679577	A comparison of the  K D values for bivalent scFv binding with BSA-A-trisaccharide  versus monovalent trisaccharide binding to scFv indicated that the avidity gain afforded by bivalency was ~75-fold for the L(103H)I and L(103H)V mutants.	bind
40672	3	9539	7	10	NULL	0	NULL	scFv		bivalent;;mutant	increase			L(103H)I		statement 1		avidity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2059_s_144	11679577	A comparison of the  K D values for bivalent scFv binding with BSA-A-trisaccharide  versus monovalent trisaccharide binding to scFv indicated that the avidity gain afforded by bivalency was ~75-fold for the L(103H)I and L(103H)V mutants.	bind
40673	4	9539	7	10	NULL	0	NULL	scFv		bivalent;;mutant	increase			 L(103H)V		statement 1		avidity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2059_s_144	11679577	A comparison of the  K D values for bivalent scFv binding with BSA-A-trisaccharide  versus monovalent trisaccharide binding to scFv indicated that the avidity gain afforded by bivalency was ~75-fold for the L(103H)I and L(103H)V mutants.	bind
41474	1	9541	5	13	NULL	NULL	NULL	cyt 	GP		bind		exclusively	b6 subunit		complex	GP	all pigments of			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1506_1_55_s_226	11418097	A comparison of the absorbance spectra and the pigment analyses of all protein-containing fractions obtained from anion exchange HPLC indicates that the cyt  b6 subunit exclusively binds all pigments of the complex.	bind
40677	1	9541	7	NULL	NULL	0	NULL	cyt	NULL		binds	NULL	exclusively	b6 subunit		complex	NULL	pigments of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1506_1_55_s_226	11418097	A comparison of the absorbance spectra and the pigment analyses of all protein-containing fractions obtained from anion exchange HPLC indicates that the cyt  b6 subunit exclusively binds all pigments of the complex.	bind
41722	1	9543	5	13	NULL	NULL	NULL	CheY	GP		is involved in			amino acid side chains		metal	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_febslett_441_2_242_s_165	9883892	A comparison of the amino acid side chains involved in metal binding between CheY and PhoB reveals that they are identical except for the substitution of a glutamate residue at position 9 of PhoB which corresponds to Asp-12 of CheY [ 15,  32].	bind
41725	2	9543	5	13	NULL	NULL	NULL	PhoB	GP		is involved in			amino acid side chains		metal	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_febslett_441_2_242_s_165	9883892	A comparison of the amino acid side chains involved in metal binding between CheY and PhoB reveals that they are identical except for the substitution of a glutamate residue at position 9 of PhoB which corresponds to Asp-12 of CheY [ 15,  32].	bind
41726	3	9543	5	13	NULL	NULL	NULL	statement 1	Process		is identical to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_441_2_242_s_165	9883892	A comparison of the amino acid side chains involved in metal binding between CheY and PhoB reveals that they are identical except for the substitution of a glutamate residue at position 9 of PhoB which corresponds to Asp-12 of CheY [ 15,  32].	bind
41729	4	9543	5	13	NULL	NULL	NULL	PhoB	GP	substitution of	corresponds to			glutamate residue at position 9		CheY	GP		Asp-12		NULL		NULL	NULL	NULL	NULL	gw60_febslett_441_2_242_s_165	9883892	A comparison of the amino acid side chains involved in metal binding between CheY and PhoB reveals that they are identical except for the substitution of a glutamate residue at position 9 of PhoB which corresponds to Asp-12 of CheY [ 15,  32].	bind
41730	5	9543	5	13	NULL	NULL	NULL	statement 4	Process		is an exception for					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_441_2_242_s_165	9883892	A comparison of the amino acid side chains involved in metal binding between CheY and PhoB reveals that they are identical except for the substitution of a glutamate residue at position 9 of PhoB which corresponds to Asp-12 of CheY [ 15,  32].	bind
40680	1	9543	7	NULL	NULL	0	NULL	CheY	NULL		bind	NULL		amino acid side chain		metal	NULL				NULL		NULL	NULL	NULL	NULL	gw60_febslett_441_2_242_s_165	9883892	A comparison of the amino acid side chains involved in metal binding between CheY and PhoB reveals that they are identical except for the substitution of a glutamate residue at position 9 of PhoB which corresponds to Asp-12 of CheY [ 15,  32].	bind
40681	2	9543	7	NULL	NULL	0	NULL	PhoB	NULL		bind	NULL		amino acid side chain		metal	NULL				NULL		NULL	NULL	NULL	NULL	gw60_febslett_441_2_242_s_165	9883892	A comparison of the amino acid side chains involved in metal binding between CheY and PhoB reveals that they are identical except for the substitution of a glutamate residue at position 9 of PhoB which corresponds to Asp-12 of CheY [ 15,  32].	bind
40682	3	9543	7	NULL	NULL	0	NULL	PhoB	NULL		differs as	NULL		glutamate residue at position 9		CheY	NULL		Asp-12		NULL		NULL	NULL	NULL	NULL	gw60_febslett_441_2_242_s_165	9883892	A comparison of the amino acid side chains involved in metal binding between CheY and PhoB reveals that they are identical except for the substitution of a glutamate residue at position 9 of PhoB which corresponds to Asp-12 of CheY [ 15,  32].	bind
40683	4	9543	7	NULL	NULL	0	NULL	statement 1	NULL	binding of	is similar to	NULL				statement 2	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_febslett_441_2_242_s_165	9883892	A comparison of the amino acid side chains involved in metal binding between CheY and PhoB reveals that they are identical except for the substitution of a glutamate residue at position 9 of PhoB which corresponds to Asp-12 of CheY [ 15,  32].	bind
40684	5	9543	7	NULL	NULL	0	NULL	statement 4	NULL		ocurs in exception with	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_febslett_441_2_242_s_165	9883892	A comparison of the amino acid side chains involved in metal binding between CheY and PhoB reveals that they are identical except for the substitution of a glutamate residue at position 9 of PhoB which corresponds to Asp-12 of CheY [ 15,  32].	bind
41484	1	9545	5	13	NULL	NULL	NULL	E.coli helicases	GP	binding activity of	is similar to					Pseudomonas sp. helicases	GP	binding activity of			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_12_3262_s_95	11406602	A comparison of the binding activity of the  E. coliand  Pseudomonas sp. helicases by surface plasmon resonance (SPR) analysis (Figure  3H) produced similar results.	bind
41682	1	9545	7	10	NULL	0	NULL	E.coli helicases	NULL	binding activity of	is similar to	NULL				Pseudomonas sp. helicases	NULL	binding activity of 			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_12_3262_s_95	11406602	A comparison of the binding activity of the  E. coliand  Pseudomonas sp. helicases by surface plasmon resonance (SPR) analysis (Figure  3H) produced similar results.	bind
41485	1	9548	5	13	NULL	NULL	NULL	naphthalene	Chemical		bind					NDO	GP		active site		NULL		NULL	NULL	NULL	NULL	gw70_science_299_5609_1039_s_55	12586937	A comparison of the binding of  naphthalene and indole ( 22) in the active site of NDO shows that they bind similarly (fig. S4).	bind
41486	2	9548	5	13	NULL	NULL	NULL	indole	Chemical		bind					NDO	GP		active site		NULL		NULL	NULL	NULL	NULL	gw70_science_299_5609_1039_s_55	12586937	A comparison of the binding of  naphthalene and indole ( 22) in the active site of NDO shows that they bind similarly (fig. S4).	bind
41487	3	9548	5	13	NULL	NULL	NULL	statement 1	Process		similar to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_science_299_5609_1039_s_55	12586937	A comparison of the binding of  naphthalene and indole ( 22) in the active site of NDO shows that they bind similarly (fig. S4).	bind
41683	1	9548	7	NULL	NULL	0	NULL	naphthalene 	NULL		bind	NULL				NDO	NULL		active site		NULL		0	NULL	NULL	NULL	gw70_science_299_5609_1039_s_55	12586937	A comparison of the binding of  naphthalene and indole ( 22) in the active site of NDO shows that they bind similarly (fig. S4).	bind
41684	2	9548	7	NULL	NULL	0	NULL	 indole	NULL		bind	NULL				NDO	NULL		active site		NULL		0	NULL	NULL	NULL	gw70_science_299_5609_1039_s_55	12586937	A comparison of the binding of  naphthalene and indole ( 22) in the active site of NDO shows that they bind similarly (fig. S4).	bind
41685	3	9548	7	NULL	NULL	0	NULL	statement 1	NULL		is similar to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_science_299_5609_1039_s_55	12586937	A comparison of the binding of  naphthalene and indole ( 22) in the active site of NDO shows that they bind similarly (fig. S4).	bind
41488	1	9549	5	13	NULL	NULL	NULL	P12a peptide	GP		bind					protein 4.1	GP		30-kDa domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_715_s_111	7822301	A comparison of the binding of  peptides P12a and P12m to the 30-kDa domain of protein 4.1 indicated  that the substitution of alanine (RYMYAAAGTYHT) for RHK completely  abolished the association of the 30-kDa domain of protein 4.1 with  peptide P12a (data not shown).	bind
41489	2	9549	5	13	NULL	NULL	NULL	P12m peptide	GP		bind					protein 4.1	GP		30-kDa domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_715_s_111	7822301	A comparison of the binding of  peptides P12a and P12m to the 30-kDa domain of protein 4.1 indicated  that the substitution of alanine (RYMYAAAGTYHT) for RHK completely  abolished the association of the 30-kDa domain of protein 4.1 with  peptide P12a (data not shown).	bind
41490	3	9549	5	13	NULL	NULL	NULL	alanine	AminoAcid		is substituted for			RYMYAAAGTYHT		RHK	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_715_s_111	7822301	A comparison of the binding of  peptides P12a and P12m to the 30-kDa domain of protein 4.1 indicated  that the substitution of alanine (RYMYAAAGTYHT) for RHK completely  abolished the association of the 30-kDa domain of protein 4.1 with  peptide P12a (data not shown).	bind
41491	4	9549	5	13	NULL	NULL	NULL	statement 3	Process		abolishes		completely			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_715_s_111	7822301	A comparison of the binding of  peptides P12a and P12m to the 30-kDa domain of protein 4.1 indicated  that the substitution of alanine (RYMYAAAGTYHT) for RHK completely  abolished the association of the 30-kDa domain of protein 4.1 with  peptide P12a (data not shown).	bind
40761	1	9549	7	NULL	NULL	0	NULL	P12a peptide	NULL		bind	NULL				protein 4.1	NULL		30-kDa domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_2_715_s_111	7822301	A comparison of the binding of  peptides P12a and P12m to the 30-kDa domain of protein 4.1 indicated  that the substitution of alanine (RYMYAAAGTYHT) for RHK completely  abolished the association of the 30-kDa domain of protein 4.1 with  peptide P12a (data not shown).	bind
40762	2	9549	7	NULL	NULL	0	NULL	P12m peptide	NULL		bind	NULL				protein 4.1	NULL		30-kDa domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_2_715_s_111	7822301	A comparison of the binding of  peptides P12a and P12m to the 30-kDa domain of protein 4.1 indicated  that the substitution of alanine (RYMYAAAGTYHT) for RHK completely  abolished the association of the 30-kDa domain of protein 4.1 with  peptide P12a (data not shown).	bind
40763	3	9549	7	NULL	NULL	0	NULL		NULL		substituted with	NULL		RHK		Alanine	NULL		RYMYAAAGTYHT		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_2_715_s_111	7822301	A comparison of the binding of  peptides P12a and P12m to the 30-kDa domain of protein 4.1 indicated  that the substitution of alanine (RYMYAAAGTYHT) for RHK completely  abolished the association of the 30-kDa domain of protein 4.1 with  peptide P12a (data not shown).	bind
40764	4	9549	7	NULL	NULL	0	NULL	statement 3	NULL		abolishes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_2_715_s_111	7822301	A comparison of the binding of  peptides P12a and P12m to the 30-kDa domain of protein 4.1 indicated  that the substitution of alanine (RYMYAAAGTYHT) for RHK completely  abolished the association of the 30-kDa domain of protein 4.1 with  peptide P12a (data not shown).	bind
41493	1	9550	5	13	NULL	NULL	NULL	L1 sequence	GP		bind					RTP dimers	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_12_8771_s_121	11124956	A comparison of the binding profiles of L1 with L1 core supports the conclusion that the complete L1 sequence bound to two dimers RTP.	bind
40765	1	9550	7	10	NULL	0	NULL	L1 sequence			bind					dimers RTP					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_12_8771_s_121	11124956	A comparison of the binding profiles of L1 with L1 core supports the conclusion that the complete L1 sequence bound to two dimers RTP.	bind
41494	1	9551	5	13	NULL	NULL	NULL	AP-1	GP		bind					CD-MPR	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_22_23542_s_40	15044437	A comparison of the binding properties of AP-1 and GGA1 to the CD-MPR revealed subtle but essential differences.	bind
41495	2	9551	5	13	NULL	NULL	NULL	GGA1	GP		bind					CD-MPR	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_22_23542_s_40	15044437	A comparison of the binding properties of AP-1 and GGA1 to the CD-MPR revealed subtle but essential differences.	bind
40766	1	9551	7	NULL	NULL	0	NULL	AP-1	NULL		bind	NULL				CD-MPR	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_22_23542_s_40	15044437	A comparison of the binding properties of AP-1 and GGA1 to the CD-MPR revealed subtle but essential differences.	bind
40767	2	9551	7	NULL	NULL	0	NULL	 GGA1	NULL		bind	NULL				CD-MPR	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_22_23542_s_40	15044437	A comparison of the binding properties of AP-1 and GGA1 to the CD-MPR revealed subtle but essential differences.	bind
41497	1	9553	5	13	NULL	NULL	NULL				bind			Y782F		ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_6_3446_s_212	9920889	A comparison of the chemical quench and pulse-chase results indicates that Y782F binds two ATP with a high commitment for catalysis, just as the wild type enzyme.	bind
41498	2	9553	5	13	NULL	NULL	NULL	statement 1	Process		commitment for		high			catalysis	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_6_3446_s_212	9920889	A comparison of the chemical quench and pulse-chase results indicates that Y782F binds two ATP with a high commitment for catalysis, just as the wild type enzyme.	bind
40774	1	9553	7	NULL	NULL	0	NULL		NULL		binds	NULL		 Y782F		ATP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_6_3446_s_212	9920889	A comparison of the chemical quench and pulse-chase results indicates that Y782F binds two ATP with a high commitment for catalysis, just as the wild type enzyme.	bind
40775	2	9553	7	10	NULL	0	NULL	statement 1	NULL		commitment for	NULL	high 			catalysis	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_6_3446_s_212	9920889	A comparison of the chemical quench and pulse-chase results indicates that Y782F binds two ATP with a high commitment for catalysis, just as the wild type enzyme.	bind
41500	1	9554	5	13	NULL	NULL	NULL	U1-A	GP		bind			N-terminal RRM		U1	GP		SLII		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_17_3057_s_240	16096647	A comparison of the cocrystals of the N-terminal RRM of U1-A and U2-B"` bound  to U1 SLII and U2 SLIV, respectively, indicates that snRNA discrimination by U1-A  and U2-B"` is the result of the formation of a different network of multiple  hydrogen-bonding interactions between the RNA and protein (  et al;   et al).	bind
41501	2	9554	5	13	NULL	NULL	NULL	U2-B	GP		bind			N-terminal RRM		U2	GP		SLIV		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_17_3057_s_240	16096647	A comparison of the cocrystals of the N-terminal RRM of U1-A and U2-B"` bound  to U1 SLII and U2 SLIV, respectively, indicates that snRNA discrimination by U1-A  and U2-B"` is the result of the formation of a different network of multiple  hydrogen-bonding interactions between the RNA and protein (  et al;   et al).	bind
41502	3	9554	5	13	NULL	NULL	NULL	U1-A	GP		discriminates					snRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_17_3057_s_240	16096647	A comparison of the cocrystals of the N-terminal RRM of U1-A and U2-B"` bound  to U1 SLII and U2 SLIV, respectively, indicates that snRNA discrimination by U1-A  and U2-B"` is the result of the formation of a different network of multiple  hydrogen-bonding interactions between the RNA and protein (  et al;   et al).	bind
41503	4	9554	5	13	NULL	NULL	NULL	U2-B	GP		discriminates					snRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_17_3057_s_240	16096647	A comparison of the cocrystals of the N-terminal RRM of U1-A and U2-B"` bound  to U1 SLII and U2 SLIV, respectively, indicates that snRNA discrimination by U1-A  and U2-B"` is the result of the formation of a different network of multiple  hydrogen-bonding interactions between the RNA and protein (  et al;   et al).	bind
41504	5	9554	5	13	NULL	NULL	NULL	RNA	NucleicAcid		interact with					protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_17_3057_s_240	16096647	A comparison of the cocrystals of the N-terminal RRM of U1-A and U2-B"` bound  to U1 SLII and U2 SLIV, respectively, indicates that snRNA discrimination by U1-A  and U2-B"` is the result of the formation of a different network of multiple  hydrogen-bonding interactions between the RNA and protein (  et al;   et al).	bind
41505	6	9554	5	13	NULL	NULL	NULL	statement 5	Process		forms					multiple hydrogen-bonding interactions	Process	different network of			NULL		NULL	NULL	NULL	NULL	gw70_embo_24_17_3057_s_240	16096647	A comparison of the cocrystals of the N-terminal RRM of U1-A and U2-B"` bound  to U1 SLII and U2 SLIV, respectively, indicates that snRNA discrimination by U1-A  and U2-B"` is the result of the formation of a different network of multiple  hydrogen-bonding interactions between the RNA and protein (  et al;   et al).	bind
41506	7	9554	5	13	NULL	NULL	NULL	statement 6	Process		results in					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_17_3057_s_240	16096647	A comparison of the cocrystals of the N-terminal RRM of U1-A and U2-B"` bound  to U1 SLII and U2 SLIV, respectively, indicates that snRNA discrimination by U1-A  and U2-B"` is the result of the formation of a different network of multiple  hydrogen-bonding interactions between the RNA and protein (  et al;   et al).	bind
41507	8	9554	5	13	NULL	NULL	NULL	statement 6	Process		results in					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_17_3057_s_240	16096647	A comparison of the cocrystals of the N-terminal RRM of U1-A and U2-B"` bound  to U1 SLII and U2 SLIV, respectively, indicates that snRNA discrimination by U1-A  and U2-B"` is the result of the formation of a different network of multiple  hydrogen-bonding interactions between the RNA and protein (  et al;   et al).	bind
40776	1	9554	7	NULL	NULL	0	NULL	U1-A	NULL		bind	NULL		N-terminal RRM		 U1 SLII	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_24_17_3057_s_240	16096647	A comparison of the cocrystals of the N-terminal RRM of U1-A and U2-B"` bound  to U1 SLII and U2 SLIV, respectively, indicates that snRNA discrimination by U1-A  and U2-B"` is the result of the formation of a different network of multiple  hydrogen-bonding interactions between the RNA and protein (  et al;   et al).	bind
40777	2	9554	7	NULL	NULL	0	NULL	U2-B	NULL		bind	NULL		N-terminal RRM		U2 SLIV	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_24_17_3057_s_240	16096647	A comparison of the cocrystals of the N-terminal RRM of U1-A and U2-B"` bound  to U1 SLII and U2 SLIV, respectively, indicates that snRNA discrimination by U1-A  and U2-B"` is the result of the formation of a different network of multiple  hydrogen-bonding interactions between the RNA and protein (  et al;   et al).	bind
40779	7	9554	7	NULL	NULL	0	NULL	statement 3	NULL		is the result of	NULL				multiple hydrogen-bonding interactions 	NULL				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_17_3057_s_240	16096647	A comparison of the cocrystals of the N-terminal RRM of U1-A and U2-B"` bound  to U1 SLII and U2 SLIV, respectively, indicates that snRNA discrimination by U1-A  and U2-B"` is the result of the formation of a different network of multiple  hydrogen-bonding interactions between the RNA and protein (  et al;   et al).	bind
40780	8	9554	7	NULL	NULL	0	NULL	statement 4	NULL		is the result of	NULL				multiple hydrogen-bonding interactions 	NULL				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_17_3057_s_240	16096647	A comparison of the cocrystals of the N-terminal RRM of U1-A and U2-B"` bound  to U1 SLII and U2 SLIV, respectively, indicates that snRNA discrimination by U1-A  and U2-B"` is the result of the formation of a different network of multiple  hydrogen-bonding interactions between the RNA and protein (  et al;   et al).	bind
40781	3	9554	7	NULL	NULL	0	NULL	U1-A	NULL		discriminates	NULL				snRNA	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_24_17_3057_s_240	16096647	A comparison of the cocrystals of the N-terminal RRM of U1-A and U2-B"` bound  to U1 SLII and U2 SLIV, respectively, indicates that snRNA discrimination by U1-A  and U2-B"` is the result of the formation of a different network of multiple  hydrogen-bonding interactions between the RNA and protein (  et al;   et al).	bind
40782	4	9554	7	NULL	NULL	0	NULL	U2-B	NULL		discriminates	NULL				snRNA	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_24_17_3057_s_240	16096647	A comparison of the cocrystals of the N-terminal RRM of U1-A and U2-B"` bound  to U1 SLII and U2 SLIV, respectively, indicates that snRNA discrimination by U1-A  and U2-B"` is the result of the formation of a different network of multiple  hydrogen-bonding interactions between the RNA and protein (  et al;   et al).	bind
40783	5	9554	7	NULL	NULL	0	NULL	statement 1	NULL		indicates	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_24_17_3057_s_240	16096647	A comparison of the cocrystals of the N-terminal RRM of U1-A and U2-B"` bound  to U1 SLII and U2 SLIV, respectively, indicates that snRNA discrimination by U1-A  and U2-B"` is the result of the formation of a different network of multiple  hydrogen-bonding interactions between the RNA and protein (  et al;   et al).	bind
40786	6	9554	7	NULL	NULL	0	NULL	statement 2	NULL		indicates	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_24_17_3057_s_240	16096647	A comparison of the cocrystals of the N-terminal RRM of U1-A and U2-B"` bound  to U1 SLII and U2 SLIV, respectively, indicates that snRNA discrimination by U1-A  and U2-B"` is the result of the formation of a different network of multiple  hydrogen-bonding interactions between the RNA and protein (  et al;   et al).	bind
41508	1	9555	5	13	NULL	NULL	NULL	SptP	GP		bind					Rac1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_6_1449_s_173	11163217	A comparison of the crystal structure of the SptP monomer with that of SptP bound to Rac1 reveals marked structural changes.	bind
40788	1	9555	7	NULL	NULL	0	NULL	SptP	NULL		bind	NULL				Rac1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_6_6_1449_s_173	11163217	A comparison of the crystal structure of the SptP monomer with that of SptP bound to Rac1 reveals marked structural changes.	bind
41509	1	9556	5	13	NULL	NULL	NULL	CFR	GP		bind					FGFs	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_5167_s_244	9030584	A comparison of the crystal structures for FGFR and CFR bound to FGFs will aid in the elucidation of the role(s) of CFR in FGF action.	bind
46866	2	9556	5	13	NULL	NULL	NULL	FGF	GP		bind					FGFR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_5167_s_244	9030584	A comparison of the crystal structures for FGFR and CFR bound to FGFs will aid in the elucidation of the role(s) of CFR in FGF action.	bind
40789	1	9556	7	NULL	NULL	0	NULL	FGFs	NULL		bind	NULL				FGFR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_8_5167_s_244	9030584	A comparison of the crystal structures for FGFR and CFR bound to FGFs will aid in the elucidation of the role(s) of CFR in FGF action.	bind
40790	2	9556	7	NULL	NULL	0	NULL	FGFs	NULL		bind	NULL				CFR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_8_5167_s_244	9030584	A comparison of the crystal structures for FGFR and CFR bound to FGFs will aid in the elucidation of the role(s) of CFR in FGF action.	bind
41510	1	9557	5	13	NULL	NULL	NULL	C/EBP	GP		is a type of					bZip protein	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_nucleic-acids-res_23_20_7479080_s_1	7479080	A comparison of the different DNA binding specificities of the bZip proteins C/EBP and GCN4..	bind
41511	2	9557	5	13	NULL	NULL	NULL	GCN4	GP		is a type of					bZip protein	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_nucleic-acids-res_23_20_7479080_s_1	7479080	A comparison of the different DNA binding specificities of the bZip proteins C/EBP and GCN4..	bind
41512	3	9557	5	13	NULL	NULL	NULL	C/EBP	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_nucleic-acids-res_23_20_7479080_s_1	7479080	A comparison of the different DNA binding specificities of the bZip proteins C/EBP and GCN4..	bind
41513	4	9557	5	13	NULL	NULL	NULL	GCN4	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_nucleic-acids-res_23_20_7479080_s_1	7479080	A comparison of the different DNA binding specificities of the bZip proteins C/EBP and GCN4..	bind
40791	1	9557	7	NULL	NULL	0	NULL	C/EBP	NULL		binds	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_nucleic-acids-res_23_20_7479080_s_1	7479080	A comparison of the different DNA binding specificities of the bZip proteins C/EBP and GCN4..	bind
40792	2	9557	7	NULL	NULL	0	NULL	GCN4	NULL		binds	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_nucleic-acids-res_23_20_7479080_s_1	7479080	A comparison of the different DNA binding specificities of the bZip proteins C/EBP and GCN4..	bind
40793	3	9557	7	NULL	NULL	0	NULL	 C/EBP 	NULL		is a type of	NULL				bZip proteins	NULL				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_nucleic-acids-res_23_20_7479080_s_1	7479080	A comparison of the different DNA binding specificities of the bZip proteins C/EBP and GCN4..	bind
40794	4	9557	7	NULL	NULL	0	NULL	GCN4	NULL		is a type of	NULL				bZip proteins	NULL				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_nucleic-acids-res_23_20_7479080_s_1	7479080	A comparison of the different DNA binding specificities of the bZip proteins C/EBP and GCN4..	bind
41514	1	9558	5	13	NULL	NULL	NULL	aflatoxin	Chemical		bind					DNA	NucleicAcid	liver			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_cancer-res_52_2_1728400_s_9	1728400	A comparison of the dose-dependent residual levels of aflatoxin  binding to liver DNA with the amount of aflatoxin-N7-guanine excreted  in urine showed a correlation coefficient of 0.98.	bind
40795	1	9558	7	NULL	NULL	0	NULL	aflatoxin	NULL		bind	NULL				liver DNA	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_cancer-res_52_2_1728400_s_9	1728400	A comparison of the dose-dependent residual levels of aflatoxin  binding to liver DNA with the amount of aflatoxin-N7-guanine excreted  in urine showed a correlation coefficient of 0.98.	bind
41516	1	9560	5	13	NULL	NULL	NULL	FKBP12	GP		bind					FK506	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_96_3_425_s_172	10025408	A Comparison of the FKBP12 - FK506  and FKBP12 - TbetaR-I Complexes A surface representation of FKBP12 bound to FK506 is shown  to the left (Wilson et al., 1995   ).	bind
41517	2	9560	5	13	NULL	NULL	NULL	FKBP12	GP		bind					TbetaR-I	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_96_3_425_s_172	10025408	A Comparison of the FKBP12 - FK506  and FKBP12 - TbetaR-I Complexes A surface representation of FKBP12 bound to FK506 is shown  to the left (Wilson et al., 1995   ).	bind
40797	1	9560	7	NULL	NULL	0	NULL	FKBP12	NULL		complex with	NULL				FK506	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cell_96_3_425_s_172	10025408	A Comparison of the FKBP12 - FK506  and FKBP12 - TbetaR-I Complexes A surface representation of FKBP12 bound to FK506 is shown  to the left (Wilson et al., 1995   ).	bind
40798	2	9560	7	NULL	NULL	0	NULL	FKBP12	NULL		complex with	NULL				TbetaR-I	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_96_3_425_s_172	10025408	A Comparison of the FKBP12 - FK506  and FKBP12 - TbetaR-I Complexes A surface representation of FKBP12 bound to FK506 is shown  to the left (Wilson et al., 1995   ).	bind
41518	1	9561	5	13	NULL	NULL	NULL	P450s	GP		is involved in					trichothecene biosynthetic pathway	Process				NULL		NULL	NULL	NULL	NULL	gw70_applenvironmicrob_70_4_2044_s_235	15066795	A comparison of the heme-binding motifs of several different P450s involved in the trichothecene biosynthetic pathway from  F. sporotrichioides and  F. graminearum shows the conservation of residues in this 20-amino-acid region.	bind
41519	2	9561	5	13	NULL	NULL	NULL	P450s	GP	F. sporotrichioides	conserved in			heme-binding motif		P450s	GP	F. graminearum	heme-binding motif		NULL		NULL	NULL	NULL	NULL	gw70_applenvironmicrob_70_4_2044_s_235	15066795	A comparison of the heme-binding motifs of several different P450s involved in the trichothecene biosynthetic pathway from  F. sporotrichioides and  F. graminearum shows the conservation of residues in this 20-amino-acid region.	bind
40800	1	9561	7	10	NULL	0	NULL	P450s			is involved in			 heme-binding motif		trichothecene biosynthetic pathway					NULL		NULL	NULL	NULL	NULL	gw70_applenvironmicrob_70_4_2044_s_235	15066795	A comparison of the heme-binding motifs of several different P450s involved in the trichothecene biosynthetic pathway from  F. sporotrichioides and  F. graminearum shows the conservation of residues in this 20-amino-acid region.	bind
40802	2	9561	7	10	NULL	0	NULL	P450s		F. sporotrichioides	is conserved with			20-amino-acid region heme-binding motif		P450s		 F. graminearum 	20-amino-acid region heme-binding motif		NULL		NULL	NULL	NULL	NULL	gw70_applenvironmicrob_70_4_2044_s_235	15066795	A comparison of the heme-binding motifs of several different P450s involved in the trichothecene biosynthetic pathway from  F. sporotrichioides and  F. graminearum shows the conservation of residues in this 20-amino-acid region.	bind
41710	1	9562	5	13	NULL	NULL	NULL	Fim3	GP		is a type of					fimbrial subunit	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_5_2256_s_10	9573115	A comparison of the heparin binding regions of Fim2 with homologous regions of Fim3 and FimX, two closely related but antigenically distinct fimbrial subunits, showed that basic amino acids and tyrosines are generally conserved.	bind
41711	2	9562	5	13	NULL	NULL	NULL	FimX	GP		is a type of					fimbrial subunit	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_5_2256_s_10	9573115	A comparison of the heparin binding regions of Fim2 with homologous regions of Fim3 and FimX, two closely related but antigenically distinct fimbrial subunits, showed that basic amino acids and tyrosines are generally conserved.	bind
41712	3	9562	5	13	NULL	NULL	NULL	Fim3	GP		is related to		closely			FimX	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_5_2256_s_10	9573115	A comparison of the heparin binding regions of Fim2 with homologous regions of Fim3 and FimX, two closely related but antigenically distinct fimbrial subunits, showed that basic amino acids and tyrosines are generally conserved.	bind
41713	4	9562	5	13	NULL	NULL	NULL	Fim3	GP		is distinct from		antigenically			FimX	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_5_2256_s_10	9573115	A comparison of the heparin binding regions of Fim2 with homologous regions of Fim3 and FimX, two closely related but antigenically distinct fimbrial subunits, showed that basic amino acids and tyrosines are generally conserved.	bind
41716	5	9562	5	13	NULL	NULL	NULL	Fim2	GP		is conserved in			basic amino acids in heparin binding regions		Fim3	GP		heparin binding regions		NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_5_2256_s_10	9573115	A comparison of the heparin binding regions of Fim2 with homologous regions of Fim3 and FimX, two closely related but antigenically distinct fimbrial subunits, showed that basic amino acids and tyrosines are generally conserved.	bind
41717	6	9562	5	13	NULL	NULL	NULL	Fim2	GP		is conserved in			basic amino acids in heparin binding regions		FimX	GP		heparin binding regions		NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_5_2256_s_10	9573115	A comparison of the heparin binding regions of Fim2 with homologous regions of Fim3 and FimX, two closely related but antigenically distinct fimbrial subunits, showed that basic amino acids and tyrosines are generally conserved.	bind
41718	7	9562	5	13	NULL	NULL	NULL	Fim2	GP		is conserved in			tyrosines in heparin binding regions		Fim3	GP		heparin binding regions		NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_5_2256_s_10	9573115	A comparison of the heparin binding regions of Fim2 with homologous regions of Fim3 and FimX, two closely related but antigenically distinct fimbrial subunits, showed that basic amino acids and tyrosines are generally conserved.	bind
41719	8	9562	5	13	NULL	NULL	NULL	Fim2	GP		is conserved in			tyrosines in heparin binding regions		FimX	GP		heparin binding regions		NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_5_2256_s_10	9573115	A comparison of the heparin binding regions of Fim2 with homologous regions of Fim3 and FimX, two closely related but antigenically distinct fimbrial subunits, showed that basic amino acids and tyrosines are generally conserved.	bind
40821	1	9562	7	NULL	NULL	0	NULL	Fim2	NULL		is conserved with	NULL		basic amino acid in heparin binding region		Fim3	NULL		basic amino acid in heparin binding region		NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_5_2256_s_10	9573115	A comparison of the heparin binding regions of Fim2 with homologous regions of Fim3 and FimX, two closely related but antigenically distinct fimbrial subunits, showed that basic amino acids and tyrosines are generally conserved.	bind
40822	2	9562	7	NULL	NULL	0	NULL	Fim2	NULL		is conserved with	NULL		basic amino acid in heparin binding region 		FimX	NULL		basic amino acid in heparin binding region 		NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_5_2256_s_10	9573115	A comparison of the heparin binding regions of Fim2 with homologous regions of Fim3 and FimX, two closely related but antigenically distinct fimbrial subunits, showed that basic amino acids and tyrosines are generally conserved.	bind
46962	3	9562	7	NULL	NULL	0	NULL	Fim2	NULL		is conserved with	NULL		tyrosine in heparin binding region		Fim3	NULL		tyrosine in heparin binding region		NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_5_2256_s_10	9573115	A comparison of the heparin binding regions of Fim2 with homologous regions of Fim3 and FimX, two closely related but antigenically distinct fimbrial subunits, showed that basic amino acids and tyrosines are generally conserved.	bind
46963	4	9562	7	NULL	NULL	0	NULL	Fim2	NULL		is conserved with	NULL		tyrosine in heparin binding region		FimX	NULL		tyrosine in heparin binding region		NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_5_2256_s_10	9573115	A comparison of the heparin binding regions of Fim2 with homologous regions of Fim3 and FimX, two closely related but antigenically distinct fimbrial subunits, showed that basic amino acids and tyrosines are generally conserved.	bind
46964	5	9562	7	NULL	NULL	0	NULL	Fim3	NULL		is a type of	NULL				fimbrial subunit	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_5_2256_s_10	9573115	A comparison of the heparin binding regions of Fim2 with homologous regions of Fim3 and FimX, two closely related but antigenically distinct fimbrial subunits, showed that basic amino acids and tyrosines are generally conserved.	bind
46965	6	9562	7	NULL	NULL	0	NULL	FimX	NULL		is a type of	NULL				fimbrial subunit	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_5_2256_s_10	9573115	A comparison of the heparin binding regions of Fim2 with homologous regions of Fim3 and FimX, two closely related but antigenically distinct fimbrial subunits, showed that basic amino acids and tyrosines are generally conserved.	bind
46966	7	9562	7	NULL	NULL	0	NULL	Fim3	NULL		related to	NULL	closely			FimX	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_5_2256_s_10	9573115	A comparison of the heparin binding regions of Fim2 with homologous regions of Fim3 and FimX, two closely related but antigenically distinct fimbrial subunits, showed that basic amino acids and tyrosines are generally conserved.	bind
46967	8	9562	7	NULL	NULL	0	NULL	Fim3	NULL		is distinct from	NULL	antigenically			FimX	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_5_2256_s_10	9573115	A comparison of the heparin binding regions of Fim2 with homologous regions of Fim3 and FimX, two closely related but antigenically distinct fimbrial subunits, showed that basic amino acids and tyrosines are generally conserved.	bind
41521	1	9564	5	13	NULL	NULL	NULL	H3	GP	hyperacetylated	bind					betaA-globin DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_37_34810_s_175	11435438	A comparison of the hybridization signal intensities of the three probes in the input and acetylated H3-immunoprecipitated DNA fractions showed that hyperacetylated H3 was bound to betaA-globin and epsilon-globin DNA but not to vitellogenin DNA.	bind
41522	2	9564	5	13	NULL	NULL	NULL	H3	GP	hyperacetylated	bind					epsilon-globin DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_37_34810_s_175	11435438	A comparison of the hybridization signal intensities of the three probes in the input and acetylated H3-immunoprecipitated DNA fractions showed that hyperacetylated H3 was bound to betaA-globin and epsilon-globin DNA but not to vitellogenin DNA.	bind
41523	3	9564	5	13	NULL	NULL	NULL	H3	GP	hyperacetylated	does not bind					vitellogenin DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_37_34810_s_175	11435438	A comparison of the hybridization signal intensities of the three probes in the input and acetylated H3-immunoprecipitated DNA fractions showed that hyperacetylated H3 was bound to betaA-globin and epsilon-globin DNA but not to vitellogenin DNA.	bind
40829	1	9564	7	10	NULL	0	NULL	betaA-globin 			bind					H3		 hyperacetylated			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_37_34810_s_175	11435438	A comparison of the hybridization signal intensities of the three probes in the input and acetylated H3-immunoprecipitated DNA fractions showed that hyperacetylated H3 was bound to betaA-globin and epsilon-globin DNA but not to vitellogenin DNA.	bind
40831	2	9564	7	10	NULL	0	NULL	H3		hyperacetylated 	bind					epsilon-globin DNA					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_37_34810_s_175	11435438	A comparison of the hybridization signal intensities of the three probes in the input and acetylated H3-immunoprecipitated DNA fractions showed that hyperacetylated H3 was bound to betaA-globin and epsilon-globin DNA but not to vitellogenin DNA.	bind
40832	3	9564	7	10	NULL	0	NULL	H3		hyperacetylated 	does not bind					vitellogenin DNA					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_37_34810_s_175	11435438	A comparison of the hybridization signal intensities of the three probes in the input and acetylated H3-immunoprecipitated DNA fractions showed that hyperacetylated H3 was bound to betaA-globin and epsilon-globin DNA but not to vitellogenin DNA.	bind
41524	1	9565	5	13	NULL	NULL	NULL	MMP-2C	GP		complex with			inhibitor binding pocket		SC-74020	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1598_1_10_s_274	12147339	A comparison of the inhibitor binding pocket of the MMP-2C solution structure (magenta) and the MMP-8 crystal structure (purple) complexed to SC-74020.	bind
41525	2	9565	5	13	NULL	NULL	NULL	MMP-8	GP		complex with			inhibitor binding pocket		SC-74020	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1598_1_10_s_274	12147339	A comparison of the inhibitor binding pocket of the MMP-2C solution structure (magenta) and the MMP-8 crystal structure (purple) complexed to SC-74020.	bind
40833	1	9565	7	NULL	NULL	0	NULL	MMP-2C	NULL		complex with	NULL		inhibitor binding pocket		SC-74020	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1598_1_10_s_274	12147339	A comparison of the inhibitor binding pocket of the MMP-2C solution structure (magenta) and the MMP-8 crystal structure (purple) complexed to SC-74020.	bind
40834	2	9565	7	NULL	NULL	0	NULL	MMP-8 	NULL		complex with	NULL		inhibitor binding pocket		SC-74020	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1598_1_10_s_274	12147339	A comparison of the inhibitor binding pocket of the MMP-2C solution structure (magenta) and the MMP-8 crystal structure (purple) complexed to SC-74020.	bind
41751	1	9566	5	13	NULL	NULL	NULL	QacR	GP		is a type of					repressor protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_611	12456787	A comparison of the ligand-binding domains of the QacR repressor and BmrR activator proteins reveals that although that of QacR is completely helical in nature ( ), whereas BmrR is predominantly beta-sheet ( ), the two proteins have notable similarities, including the aromatic, hydrophobic, and negatively charged residues that line their binding pockets as well as the crucial role played by tyrosines (see below).	bind
41752	2	9566	5	13	NULL	NULL	NULL	BmrR	GP		is a type of					activator protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_611	12456787	A comparison of the ligand-binding domains of the QacR repressor and BmrR activator proteins reveals that although that of QacR is completely helical in nature ( ), whereas BmrR is predominantly beta-sheet ( ), the two proteins have notable similarities, including the aromatic, hydrophobic, and negatively charged residues that line their binding pockets as well as the crucial role played by tyrosines (see below).	bind
41754	3	9566	5	13	NULL	NULL	NULL	QacR	GP		exhibits			ligand-binding domain		helical structure	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_611	12456787	A comparison of the ligand-binding domains of the QacR repressor and BmrR activator proteins reveals that although that of QacR is completely helical in nature ( ), whereas BmrR is predominantly beta-sheet ( ), the two proteins have notable similarities, including the aromatic, hydrophobic, and negatively charged residues that line their binding pockets as well as the crucial role played by tyrosines (see below).	bind
41760	4	9566	5	13	NULL	NULL	NULL	BmrR	GP		exhibits			ligand-binding domain		beta-sheet structure	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_611	12456787	A comparison of the ligand-binding domains of the QacR repressor and BmrR activator proteins reveals that although that of QacR is completely helical in nature ( ), whereas BmrR is predominantly beta-sheet ( ), the two proteins have notable similarities, including the aromatic, hydrophobic, and negatively charged residues that line their binding pockets as well as the crucial role played by tyrosines (see below).	bind
41761	5	9566	5	13	NULL	NULL	NULL	QacR	GP		is similar to			aromatic;;hydrophobic;;negatively charged residues		BmrR	GP		aromatic;;hydrophobic;;negatively charged residues		NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_611	12456787	A comparison of the ligand-binding domains of the QacR repressor and BmrR activator proteins reveals that although that of QacR is completely helical in nature ( ), whereas BmrR is predominantly beta-sheet ( ), the two proteins have notable similarities, including the aromatic, hydrophobic, and negatively charged residues that line their binding pockets as well as the crucial role played by tyrosines (see below).	bind
41681	1	9566	7	10	NULL	0	NULL	QacR	NULL		is similar to	NULL		aromatic;;hydrophobic;;negatively charged residues		BmrR	NULL		aromatic;;hydrophobic;;negatively charged residues		NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_611	12456787	A comparison of the ligand-binding domains of the QacR repressor and BmrR activator proteins reveals that although that of QacR is completely helical in nature ( ), whereas BmrR is predominantly beta-sheet ( ), the two proteins have notable similarities, including the aromatic, hydrophobic, and negatively charged residues that line their binding pockets as well as the crucial role played by tyrosines (see below).	bind
48097	2	9566	7	10	NULL	0	NULL	QacR	NULL		is a type of	NULL				repressor	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_611	12456787	A comparison of the ligand-binding domains of the QacR repressor and BmrR activator proteins reveals that although that of QacR is completely helical in nature ( ), whereas BmrR is predominantly beta-sheet ( ), the two proteins have notable similarities, including the aromatic, hydrophobic, and negatively charged residues that line their binding pockets as well as the crucial role played by tyrosines (see below).	bind
48098	3	9566	7	10	NULL	0	NULL	BmrR	NULL		is a type of	NULL				activator	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_611	12456787	A comparison of the ligand-binding domains of the QacR repressor and BmrR activator proteins reveals that although that of QacR is completely helical in nature ( ), whereas BmrR is predominantly beta-sheet ( ), the two proteins have notable similarities, including the aromatic, hydrophobic, and negatively charged residues that line their binding pockets as well as the crucial role played by tyrosines (see below).	bind
48099	4	9566	7	10	NULL	0	NULL	QacR	NULL		exhibit	NULL		ligand-binding domain		helical structure	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_611	12456787	A comparison of the ligand-binding domains of the QacR repressor and BmrR activator proteins reveals that although that of QacR is completely helical in nature ( ), whereas BmrR is predominantly beta-sheet ( ), the two proteins have notable similarities, including the aromatic, hydrophobic, and negatively charged residues that line their binding pockets as well as the crucial role played by tyrosines (see below).	bind
48100	5	9566	7	10	NULL	0	NULL	BmrR	NULL		exhibit	NULL		ligand-binding domain		beta-sheet	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_611	12456787	A comparison of the ligand-binding domains of the QacR repressor and BmrR activator proteins reveals that although that of QacR is completely helical in nature ( ), whereas BmrR is predominantly beta-sheet ( ), the two proteins have notable similarities, including the aromatic, hydrophobic, and negatively charged residues that line their binding pockets as well as the crucial role played by tyrosines (see below).	bind
41526	1	9568	5	13	NULL	NULL	NULL	v -src	GP		bind					Cx43	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_144_5_1033_s_271	10085299	A comparison of the loss of v -src binding to Cx43 and its  functional effect on channel gating	bind
41527	2	9568	5	13	NULL	NULL	NULL	statement 1	Process	loss of	effect					channel gating	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_144_5_1033_s_271	10085299	A comparison of the loss of v -src binding to Cx43 and its  functional effect on channel gating	bind
40840	1	9568	7	NULL	NULL	0	NULL	v -src	NULL		does not bind	NULL				Cx43	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_144_5_1033_s_271	10085299	A comparison of the loss of v -src binding to Cx43 and its  functional effect on channel gating	bind
40841	2	9568	7	10	NULL	0	NULL	statement 1		loss of 	effect					channel gating					NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_144_5_1033_s_271	10085299	A comparison of the loss of v -src binding to Cx43 and its  functional effect on channel gating	bind
41534	1	9570	5	13	NULL	NULL	NULL	formate	Chemical		bind					apo-MhFbpA	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_12_3903_s_179	15175304	A comparison of the MhFbpAFeCO3 and formate-bound apo-MhFbpA structures reveals that anion-bound MhFbpA positions all of the iron-binding protein ligands within 0.5  Ang  of their positions in the ferric ion-bound state.	bind
41535	2	9570	5	13	NULL	NULL	NULL	FeCO3	Chemical		bind					MhFbpA	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_12_3903_s_179	15175304	A comparison of the MhFbpAFeCO3 and formate-bound apo-MhFbpA structures reveals that anion-bound MhFbpA positions all of the iron-binding protein ligands within 0.5  Ang  of their positions in the ferric ion-bound state.	bind
40843	1	9570	7	NULL	NULL	0	NULL	formate	NULL		bind	NULL				apo-MhFbpA	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_12_3903_s_179	15175304	A comparison of the MhFbpAFeCO3 and formate-bound apo-MhFbpA structures reveals that anion-bound MhFbpA positions all of the iron-binding protein ligands within 0.5  Ang  of their positions in the ferric ion-bound state.	bind
40844	2	9570	7	NULL	NULL	0	NULL	FeCO3	NULL		bind	NULL				MhFbpA 	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_12_3903_s_179	15175304	A comparison of the MhFbpAFeCO3 and formate-bound apo-MhFbpA structures reveals that anion-bound MhFbpA positions all of the iron-binding protein ligands within 0.5  Ang  of their positions in the ferric ion-bound state.	bind
41742	1	9571	5	13	NULL	NULL	NULL	USH-F9	GP		is similar to			NF binding faces		C32H	GP		NF binding faces		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_38_35720_s_327	12110675	A comparison of the NF binding faces of USH-F9 and C32H shows that, with the exception of the two aromatics, the binding faces are otherwise largely unperturbed.	bind
41743	2	9571	5	13	NULL	NULL	NULL	USH-F9	GP		differs from			aromatics		USH-F9	GP		NF binding face		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_38_35720_s_327	12110675	A comparison of the NF binding faces of USH-F9 and C32H shows that, with the exception of the two aromatics, the binding faces are otherwise largely unperturbed.	bind
41694	1	9571	7	NULL	NULL	0	NULL	USH-F9	NULL		is similar to	NULL		NF binding face		C32H	NULL		NF binding face		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_38_35720_s_327	12110675	A comparison of the NF binding faces of USH-F9 and C32H shows that, with the exception of the two aromatics, the binding faces are otherwise largely unperturbed.	bind
41695	2	9571	7	NULL	NULL	0	NULL	USH-F9	NULL		differs 	NULL		aromatics		C32H	NULL		aromatics		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_38_35720_s_327	12110675	A comparison of the NF binding faces of USH-F9 and C32H shows that, with the exception of the two aromatics, the binding faces are otherwise largely unperturbed.	bind
41537	1	9572	5	13	NULL	NULL	NULL	SSB1	GP		bind					ssDNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_15_3270_s_157	11470885	A comparison of the NTD with itself gave a DALI score of 24, while a comparison of the NTD with an SSB1 structure bound to ssDNA gave a DALI score of 4.1, with a root mean square difference (r.m.s.d.) in the average alpha carbon positions of 3.9  Ang .	bind
40845	1	9572	7	NULL	NULL	0	NULL	SSB1	NULL		bind	NULL				ssDNA	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_15_3270_s_157	11470885	A comparison of the NTD with itself gave a DALI score of 24, while a comparison of the NTD with an SSB1 structure bound to ssDNA gave a DALI score of 4.1, with a root mean square difference (r.m.s.d.) in the average alpha carbon positions of 3.9  Ang .	bind
41538	1	9573	5	13	NULL	NULL	NULL	scFv clones	GP		bind		irreversibly			CRA I	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_20436_s_158	12668670	A comparison of the peptide-MCA cleaving activity  (Glu-Ala-Arg-MCA substrate) and irreversible CRA  I binding by the scFv  clones indicated a strong correlation ( p < 0.005,   r2 = 0.77) ( Fig.  4 B), confirming the functional importance of superior  nucleophilic reactivity.	bind
41540	2	9573	5	13	NULL	NULL	NULL	statement 1	Process		confirms					superior nucleophilic reactivity	Process	importance of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_22_20436_s_158	12668670	A comparison of the peptide-MCA cleaving activity  (Glu-Ala-Arg-MCA substrate) and irreversible CRA  I binding by the scFv  clones indicated a strong correlation ( p < 0.005,   r2 = 0.77) ( Fig.  4 B), confirming the functional importance of superior  nucleophilic reactivity.	bind
40846	1	9573	7	NULL	NULL	0	NULL	scFv clones	NULL		bind	NULL	irreversibly			 CRA I	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_22_20436_s_158	12668670	A comparison of the peptide-MCA cleaving activity  (Glu-Ala-Arg-MCA substrate) and irreversible CRA  I binding by the scFv  clones indicated a strong correlation ( p < 0.005,   r2 = 0.77) ( Fig.  4 B), confirming the functional importance of superior  nucleophilic reactivity.	bind
40848	2	9573	7	NULL	NULL	0	NULL	statement 1	NULL		confirms	NULL				superior nucleophilic reactivity	NULL	importance of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_22_20436_s_158	12668670	A comparison of the peptide-MCA cleaving activity  (Glu-Ala-Arg-MCA substrate) and irreversible CRA  I binding by the scFv  clones indicated a strong correlation ( p < 0.005,   r2 = 0.77) ( Fig.  4 B), confirming the functional importance of superior  nucleophilic reactivity.	bind
41541	1	9574	5	13	NULL	NULL	NULL	PU.1	GP		bind					oligonucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_898_s_240	7822329	A comparison of the percentage of each oligonucleotide bound to  PU.1 indicated that PU.1 bound to the Vkappa19 pyrimidine-rich motif  with the same affinity as to the SV40 PU box, which contains a strong  binding site for PU.1, and that it had a 4 times weaker affinity to the  pyrimidine-rich motif of the V101 promoter.	bind
41542	2	9574	5	13	NULL	NULL	NULL	PU.1	GP		bind					Vkappa19	GP			pyrimidine-rich motif	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_898_s_240	7822329	A comparison of the percentage of each oligonucleotide bound to  PU.1 indicated that PU.1 bound to the Vkappa19 pyrimidine-rich motif  with the same affinity as to the SV40 PU box, which contains a strong  binding site for PU.1, and that it had a 4 times weaker affinity to the  pyrimidine-rich motif of the V101 promoter.	bind
41543	3	9574	5	13	NULL	NULL	NULL	PU.1	GP		bind					SV40	NucleicAcid			PU box	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_898_s_240	7822329	A comparison of the percentage of each oligonucleotide bound to  PU.1 indicated that PU.1 bound to the Vkappa19 pyrimidine-rich motif  with the same affinity as to the SV40 PU box, which contains a strong  binding site for PU.1, and that it had a 4 times weaker affinity to the  pyrimidine-rich motif of the V101 promoter.	bind
41544	4	9574	5	13	NULL	NULL	NULL	statement 2	Process		same affinity as					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_898_s_240	7822329	A comparison of the percentage of each oligonucleotide bound to  PU.1 indicated that PU.1 bound to the Vkappa19 pyrimidine-rich motif  with the same affinity as to the SV40 PU box, which contains a strong  binding site for PU.1, and that it had a 4 times weaker affinity to the  pyrimidine-rich motif of the V101 promoter.	bind
41545	5	9574	5	13	NULL	NULL	NULL	SV40	NucleicAcid		contains				PU box	PU.1	GP		strong binding site for		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_898_s_240	7822329	A comparison of the percentage of each oligonucleotide bound to  PU.1 indicated that PU.1 bound to the Vkappa19 pyrimidine-rich motif  with the same affinity as to the SV40 PU box, which contains a strong  binding site for PU.1, and that it had a 4 times weaker affinity to the  pyrimidine-rich motif of the V101 promoter.	bind
41546	6	9574	5	13	NULL	NULL	NULL	PU.1	GP		bind					V101	NucleicAcid			pyrimidine-rich motif of promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_898_s_240	7822329	A comparison of the percentage of each oligonucleotide bound to  PU.1 indicated that PU.1 bound to the Vkappa19 pyrimidine-rich motif  with the same affinity as to the SV40 PU box, which contains a strong  binding site for PU.1, and that it had a 4 times weaker affinity to the  pyrimidine-rich motif of the V101 promoter.	bind
41547	7	9574	5	13	NULL	NULL	NULL	statement 2	Process		weaker affinity to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_898_s_240	7822329	A comparison of the percentage of each oligonucleotide bound to  PU.1 indicated that PU.1 bound to the Vkappa19 pyrimidine-rich motif  with the same affinity as to the SV40 PU box, which contains a strong  binding site for PU.1, and that it had a 4 times weaker affinity to the  pyrimidine-rich motif of the V101 promoter.	bind
40849	1	9574	7	NULL	NULL	0	NULL	oligonucleotide	NULL		bind	NULL				PU.1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_2_898_s_240	7822329	A comparison of the percentage of each oligonucleotide bound to  PU.1 indicated that PU.1 bound to the Vkappa19 pyrimidine-rich motif  with the same affinity as to the SV40 PU box, which contains a strong  binding site for PU.1, and that it had a 4 times weaker affinity to the  pyrimidine-rich motif of the V101 promoter.	bind
40850	2	9574	7	NULL	NULL	0	NULL	PU.1	NULL		bind	NULL				 Vkappa19	NULL			pyrimidine-rich motif	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_2_898_s_240	7822329	A comparison of the percentage of each oligonucleotide bound to  PU.1 indicated that PU.1 bound to the Vkappa19 pyrimidine-rich motif  with the same affinity as to the SV40 PU box, which contains a strong  binding site for PU.1, and that it had a 4 times weaker affinity to the  pyrimidine-rich motif of the V101 promoter.	bind
40851	3	9574	7	NULL	NULL	0	NULL	 PU.1	NULL		bind	NULL				 SV40 	NULL			PU box	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_2_898_s_240	7822329	A comparison of the percentage of each oligonucleotide bound to  PU.1 indicated that PU.1 bound to the Vkappa19 pyrimidine-rich motif  with the same affinity as to the SV40 PU box, which contains a strong  binding site for PU.1, and that it had a 4 times weaker affinity to the  pyrimidine-rich motif of the V101 promoter.	bind
40852	4	9574	7	NULL	NULL	0	NULL	statement 2	NULL	affinity of	is same as	NULL				statement 3	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_2_898_s_240	7822329	A comparison of the percentage of each oligonucleotide bound to  PU.1 indicated that PU.1 bound to the Vkappa19 pyrimidine-rich motif  with the same affinity as to the SV40 PU box, which contains a strong  binding site for PU.1, and that it had a 4 times weaker affinity to the  pyrimidine-rich motif of the V101 promoter.	bind
40853	5	9574	7	10	NULL	0	NULL	 SV40 			contains				PU box	PU.1			strong binding site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_898_s_240	7822329	A comparison of the percentage of each oligonucleotide bound to  PU.1 indicated that PU.1 bound to the Vkappa19 pyrimidine-rich motif  with the same affinity as to the SV40 PU box, which contains a strong  binding site for PU.1, and that it had a 4 times weaker affinity to the  pyrimidine-rich motif of the V101 promoter.	bind
40854	6	9574	7	NULL	NULL	0	NULL	PU.1	NULL		affinity for	NULL	weaker			V101	NULL			pyrimidine-rich motif in the promotoer	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_2_898_s_240	7822329	A comparison of the percentage of each oligonucleotide bound to  PU.1 indicated that PU.1 bound to the Vkappa19 pyrimidine-rich motif  with the same affinity as to the SV40 PU box, which contains a strong  binding site for PU.1, and that it had a 4 times weaker affinity to the  pyrimidine-rich motif of the V101 promoter.	bind
43537	1	9575	5	13	NULL	NULL	NULL	apoA-I	GP	recombinant;;pro form of	bind					phospholipid transfer protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_41_11_1872_s_4	11060357	A comparison of the properties of the pro- and mature forms of recombinant apoA-I and human plasma apoA-I showed no difference between all three in their secondary structure, their ability to self-associate, lipid-binding capacity, lecithin: cholesterolacyltransferase  activation, and binding to the phospholipid transfer protein.	bind
43538	2	9575	5	13	NULL	NULL	NULL	apoA-I	GP	recombinant;;mature form of	bind					phospholipid transfer protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_41_11_1872_s_4	11060357	A comparison of the properties of the pro- and mature forms of recombinant apoA-I and human plasma apoA-I showed no difference between all three in their secondary structure, their ability to self-associate, lipid-binding capacity, lecithin: cholesterolacyltransferase  activation, and binding to the phospholipid transfer protein.	bind
43539	3	9575	5	13	NULL	NULL	NULL	apoA-I	GP	human;;plasma	bind					phospholipid transfer protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_41_11_1872_s_4	11060357	A comparison of the properties of the pro- and mature forms of recombinant apoA-I and human plasma apoA-I showed no difference between all three in their secondary structure, their ability to self-associate, lipid-binding capacity, lecithin: cholesterolacyltransferase  activation, and binding to the phospholipid transfer protein.	bind
43540	4	9575	5	13	NULL	NULL	NULL	apoA-I	GP	recombinant;;pro form of	has ability to					self-associate	Process				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_41_11_1872_s_4	11060357	A comparison of the properties of the pro- and mature forms of recombinant apoA-I and human plasma apoA-I showed no difference between all three in their secondary structure, their ability to self-associate, lipid-binding capacity, lecithin: cholesterolacyltransferase  activation, and binding to the phospholipid transfer protein.	bind
43541	5	9575	5	13	NULL	NULL	NULL	apoA-I	GP	recombinant;;mature form of	has ability to					self-associate	Process				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_41_11_1872_s_4	11060357	A comparison of the properties of the pro- and mature forms of recombinant apoA-I and human plasma apoA-I showed no difference between all three in their secondary structure, their ability to self-associate, lipid-binding capacity, lecithin: cholesterolacyltransferase  activation, and binding to the phospholipid transfer protein.	bind
43542	6	9575	5	13	NULL	NULL	NULL	apoA-I	GP	human;;plasma	has ability to					self-associate	Process				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_41_11_1872_s_4	11060357	A comparison of the properties of the pro- and mature forms of recombinant apoA-I and human plasma apoA-I showed no difference between all three in their secondary structure, their ability to self-associate, lipid-binding capacity, lecithin: cholesterolacyltransferase  activation, and binding to the phospholipid transfer protein.	bind
43543	7	9575	5	13	NULL	NULL	NULL	apoA-I	GP	recombinant;;pro form of	bind					lipid	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_41_11_1872_s_4	11060357	A comparison of the properties of the pro- and mature forms of recombinant apoA-I and human plasma apoA-I showed no difference between all three in their secondary structure, their ability to self-associate, lipid-binding capacity, lecithin: cholesterolacyltransferase  activation, and binding to the phospholipid transfer protein.	bind
43544	8	9575	5	13	NULL	NULL	NULL	apoA-I	GP	recombinant;;mature form of	bind					lipid	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_41_11_1872_s_4	11060357	A comparison of the properties of the pro- and mature forms of recombinant apoA-I and human plasma apoA-I showed no difference between all three in their secondary structure, their ability to self-associate, lipid-binding capacity, lecithin: cholesterolacyltransferase  activation, and binding to the phospholipid transfer protein.	bind
43545	9	9575	5	13	NULL	NULL	NULL	apoA-I	GP	human;;plasma	bind					lipid	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_41_11_1872_s_4	11060357	A comparison of the properties of the pro- and mature forms of recombinant apoA-I and human plasma apoA-I showed no difference between all three in their secondary structure, their ability to self-associate, lipid-binding capacity, lecithin: cholesterolacyltransferase  activation, and binding to the phospholipid transfer protein.	bind
43546	10	9575	5	13	NULL	NULL	NULL	apoA-I	GP	recombinant;;pro form of	activates					lecithin: cholesterolacyltransferase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_41_11_1872_s_4	11060357	A comparison of the properties of the pro- and mature forms of recombinant apoA-I and human plasma apoA-I showed no difference between all three in their secondary structure, their ability to self-associate, lipid-binding capacity, lecithin: cholesterolacyltransferase  activation, and binding to the phospholipid transfer protein.	bind
43547	11	9575	5	13	NULL	NULL	NULL	apoA-I	GP	recombinant;;mature form of	activates					lecithin: cholesterolacyltransferase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_41_11_1872_s_4	11060357	A comparison of the properties of the pro- and mature forms of recombinant apoA-I and human plasma apoA-I showed no difference between all three in their secondary structure, their ability to self-associate, lipid-binding capacity, lecithin: cholesterolacyltransferase  activation, and binding to the phospholipid transfer protein.	bind
43548	12	9575	5	13	NULL	NULL	NULL	apoA-I	GP	human;;plasma	activates					lecithin: cholesterolacyltransferase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_41_11_1872_s_4	11060357	A comparison of the properties of the pro- and mature forms of recombinant apoA-I and human plasma apoA-I showed no difference between all three in their secondary structure, their ability to self-associate, lipid-binding capacity, lecithin: cholesterolacyltransferase  activation, and binding to the phospholipid transfer protein.	bind
40855	1	9575	7	NULL	NULL	0	NULL	pro apoA-I	NULL	recombinant	associate with	NULL				pro apoA-I	NULL	recombinant			NULL		0	NULL	NULL	NULL	gw60_jlipidres_41_11_1872_s_4	11060357	A comparison of the properties of the pro- and mature forms of recombinant apoA-I and human plasma apoA-I showed no difference between all three in their secondary structure, their ability to self-associate, lipid-binding capacity, lecithin: cholesterolacyltransferase  activation, and binding to the phospholipid transfer protein.	bind
40856	2	9575	7	NULL	NULL	0	NULL	pro apoA-I	NULL	recombinant	bind	NULL				lipids	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_41_11_1872_s_4	11060357	A comparison of the properties of the pro- and mature forms of recombinant apoA-I and human plasma apoA-I showed no difference between all three in their secondary structure, their ability to self-associate, lipid-binding capacity, lecithin: cholesterolacyltransferase  activation, and binding to the phospholipid transfer protein.	bind
40857	3	9575	7	NULL	NULL	0	NULL	pro apoA-I	NULL	recombinant	activates	NULL				lecithin: cholesterolacyltransferase	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_41_11_1872_s_4	11060357	A comparison of the properties of the pro- and mature forms of recombinant apoA-I and human plasma apoA-I showed no difference between all three in their secondary structure, their ability to self-associate, lipid-binding capacity, lecithin: cholesterolacyltransferase  activation, and binding to the phospholipid transfer protein.	bind
40858	4	9575	7	NULL	NULL	0	NULL	pro apoA-I	NULL	recombinant	bind	NULL				phospholipid transfer protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_41_11_1872_s_4	11060357	A comparison of the properties of the pro- and mature forms of recombinant apoA-I and human plasma apoA-I showed no difference between all three in their secondary structure, their ability to self-associate, lipid-binding capacity, lecithin: cholesterolacyltransferase  activation, and binding to the phospholipid transfer protein.	bind
40859	5	9575	7	NULL	NULL	0	NULL	mature apoA-I	NULL	recombinant	associate with	NULL				mature apoA-I	NULL	recombinant			NULL		0	NULL	NULL	NULL	gw60_jlipidres_41_11_1872_s_4	11060357	A comparison of the properties of the pro- and mature forms of recombinant apoA-I and human plasma apoA-I showed no difference between all three in their secondary structure, their ability to self-associate, lipid-binding capacity, lecithin: cholesterolacyltransferase  activation, and binding to the phospholipid transfer protein.	bind
40860	6	9575	7	NULL	NULL	0	NULL	mature apoA-I	NULL	recombinant	bind	NULL				lipids	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_41_11_1872_s_4	11060357	A comparison of the properties of the pro- and mature forms of recombinant apoA-I and human plasma apoA-I showed no difference between all three in their secondary structure, their ability to self-associate, lipid-binding capacity, lecithin: cholesterolacyltransferase  activation, and binding to the phospholipid transfer protein.	bind
40861	7	9575	7	NULL	NULL	0	NULL	mature apoA-I	NULL	recombinant	activates	NULL				lecithin: cholesterolacyltransferase	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_41_11_1872_s_4	11060357	A comparison of the properties of the pro- and mature forms of recombinant apoA-I and human plasma apoA-I showed no difference between all three in their secondary structure, their ability to self-associate, lipid-binding capacity, lecithin: cholesterolacyltransferase  activation, and binding to the phospholipid transfer protein.	bind
40862	8	9575	7	NULL	NULL	0	NULL	mature apoA-I	NULL	recombinant	bind	NULL				phospholipid transfer protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_41_11_1872_s_4	11060357	A comparison of the properties of the pro- and mature forms of recombinant apoA-I and human plasma apoA-I showed no difference between all three in their secondary structure, their ability to self-associate, lipid-binding capacity, lecithin: cholesterolacyltransferase  activation, and binding to the phospholipid transfer protein.	bind
40863	9	9575	7	NULL	NULL	0	NULL	apoA-I	NULL	human plasma	associate with	NULL				apoA-I	NULL	human plasma			NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_41_11_1872_s_4	11060357	A comparison of the properties of the pro- and mature forms of recombinant apoA-I and human plasma apoA-I showed no difference between all three in their secondary structure, their ability to self-associate, lipid-binding capacity, lecithin: cholesterolacyltransferase  activation, and binding to the phospholipid transfer protein.	bind
40864	10	9575	7	NULL	NULL	0	NULL	apoA-I	NULL	human plasma	bind	NULL				lipids	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_41_11_1872_s_4	11060357	A comparison of the properties of the pro- and mature forms of recombinant apoA-I and human plasma apoA-I showed no difference between all three in their secondary structure, their ability to self-associate, lipid-binding capacity, lecithin: cholesterolacyltransferase  activation, and binding to the phospholipid transfer protein.	bind
40865	11	9575	7	NULL	NULL	0	NULL	apoA-I	NULL	human plasma	activates	NULL				lecithin: cholesterolacyltransferase	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_41_11_1872_s_4	11060357	A comparison of the properties of the pro- and mature forms of recombinant apoA-I and human plasma apoA-I showed no difference between all three in their secondary structure, their ability to self-associate, lipid-binding capacity, lecithin: cholesterolacyltransferase  activation, and binding to the phospholipid transfer protein.	bind
40867	12	9575	7	NULL	NULL	0	NULL	apoA-I	NULL	human plasma	bind	NULL				phospholipid transfer protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_41_11_1872_s_4	11060357	A comparison of the properties of the pro- and mature forms of recombinant apoA-I and human plasma apoA-I showed no difference between all three in their secondary structure, their ability to self-associate, lipid-binding capacity, lecithin: cholesterolacyltransferase  activation, and binding to the phospholipid transfer protein.	bind
41709	1	9576	5	13	NULL	NULL	NULL	RNAP	GP		bind					pRM	NucleicAcid			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_1_216_s_49	10613884	A comparison of the pseudo-first-order rate constants ( kobs) for the binding of RNAP to the pRM promoter in the context of the different deletions is graphically shown in Fig.  2a, and the values for  kobs for each promoter deletion mutant are given in Table  1.	bind
40868	1	9576	7	NULL	NULL	0	NULL	RNAP 	NULL		bind	NULL				pRM	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_1_216_s_49	10613884	A comparison of the pseudo-first-order rate constants ( kobs) for the binding of RNAP to the pRM promoter in the context of the different deletions is graphically shown in Fig.  2a, and the values for  kobs for each promoter deletion mutant are given in Table  1.	bind
41706	1	9577	5	13	NULL	NULL	NULL	ezrin	GP		is homologous to			RII binding motif		MAP2	GP		RII binding motif		NULL		NULL	NULL	NULL	NULL	gw60_embo_16_1_35_s_89	9009265	A comparison of the region spanning the RII binding motif of ezrin with analogous regions from MAP2, HT-31 and AKAP79 (Figure  6B) shows significant homologies throughout the sequence.	bind
41707	2	9577	5	13	NULL	NULL	NULL	ezrin	GP		is homologous to			RII binding motif		HT-31	GP		RII binding motif		NULL		NULL	NULL	NULL	NULL	gw60_embo_16_1_35_s_89	9009265	A comparison of the region spanning the RII binding motif of ezrin with analogous regions from MAP2, HT-31 and AKAP79 (Figure  6B) shows significant homologies throughout the sequence.	bind
41708	3	9577	5	13	NULL	NULL	NULL	ezrin	GP		is homologous to			RII binding motif		AKAP79	GP		RII binding motif		NULL		NULL	NULL	NULL	NULL	gw60_embo_16_1_35_s_89	9009265	A comparison of the region spanning the RII binding motif of ezrin with analogous regions from MAP2, HT-31 and AKAP79 (Figure  6B) shows significant homologies throughout the sequence.	bind
41700	1	9577	7	NULL	NULL	0	NULL	ezrin	NULL		is homologous to	NULL		RII binding motif		MAP2	NULL		RII binding motif		NULL		0	NULL	NULL	NULL	gw60_embo_16_1_35_s_89	9009265	A comparison of the region spanning the RII binding motif of ezrin with analogous regions from MAP2, HT-31 and AKAP79 (Figure  6B) shows significant homologies throughout the sequence.	bind
41701	2	9577	7	NULL	NULL	0	NULL	ezrin	NULL		is homologous to	NULL		RII binding motif		HT-31	NULL		RII binding motif		NULL		0	NULL	NULL	NULL	gw60_embo_16_1_35_s_89	9009265	A comparison of the region spanning the RII binding motif of ezrin with analogous regions from MAP2, HT-31 and AKAP79 (Figure  6B) shows significant homologies throughout the sequence.	bind
41702	3	9577	7	NULL	NULL	0	NULL	ezrin	NULL		is homologous to	NULL		RII binding motif		AKAP79	NULL		RII binding motif		NULL		0	NULL	NULL	NULL	gw60_embo_16_1_35_s_89	9009265	A comparison of the region spanning the RII binding motif of ezrin with analogous regions from MAP2, HT-31 and AKAP79 (Figure  6B) shows significant homologies throughout the sequence.	bind
42703	1	9578	5	13	NULL	NULL	NULL	WASP	GP		bind		preferentially			Cdc42	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_47_36999_s_106	10950951	A comparison of the relative amounts of active Rac and active Cdc42 with the total amounts of the GTPases (Fig.  1 A) is consistent with WASP preferentially binding Cdc42 over Rac ( 12,  23).	bind
42704	2	9578	5	13	NULL	NULL	NULL	WASP	GP		bind					Rac	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_47_36999_s_106	10950951	A comparison of the relative amounts of active Rac and active Cdc42 with the total amounts of the GTPases (Fig.  1 A) is consistent with WASP preferentially binding Cdc42 over Rac ( 12,  23).	bind
40869	1	9578	7	NULL	NULL	0	NULL	WASP	NULL		bind	NULL	preferentially			Cdc42	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_47_36999_s_106	10950951	A comparison of the relative amounts of active Rac and active Cdc42 with the total amounts of the GTPases (Fig.  1 A) is consistent with WASP preferentially binding Cdc42 over Rac ( 12,  23).	bind
40870	2	9578	7	NULL	NULL	0	NULL	WASP	NULL		bind	NULL				Rac	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_47_36999_s_106	10950951	A comparison of the relative amounts of active Rac and active Cdc42 with the total amounts of the GTPases (Fig.  1 A) is consistent with WASP preferentially binding Cdc42 over Rac ( 12,  23).	bind
42706	1	9579	5	13	NULL	NULL	NULL	SarR	GP		bind					sar	NucleicAcid			P1 promoter	NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_2_885_s_217	11159982	A comparison of the relative binding of SarR and SarA to the  sar P1 promoter is of interest.	bind
42707	2	9579	5	13	NULL	NULL	NULL	SarA	GP		bind					sar	NucleicAcid			P1 promoter	NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_2_885_s_217	11159982	A comparison of the relative binding of SarR and SarA to the  sar P1 promoter is of interest.	bind
40871	1	9579	7	10	NULL	0	NULL	SarR	NULL		bind	NULL				sar 	NULL			P1 promoter	NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_2_885_s_217	11159982	A comparison of the relative binding of SarR and SarA to the  sar P1 promoter is of interest.	bind
40872	2	9579	7	10	NULL	0	NULL	SarA	NULL		bind	NULL				sar	NULL			P1 promoter	NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_2_885_s_217	11159982	A comparison of the relative binding of SarR and SarA to the  sar P1 promoter is of interest.	bind
42791	1	9582	5	13	NULL	NULL	NULL			mutation of	does not effect		grossly	D140A		alpha4beta7	GP	structure of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_33_25652_s_232	10837471	A comparison of the staining obtained with mAbs to at least two different epitopes on the alpha4 chain (B5G10, B5E2, and HP1/2) ( 76), three different epitopes on the beta7 chain (Fib21, Fib30, and Fib504) ( 65), and an antibody that recognizes cell-surface beta7 chain only in the context of alpha4beta7 (ACT-1) ( 60,  77) showed that the binding of these mAbs was unaffected and confirmed that the D140A mutation did not grossly affect the structure of alpha4beta7 (Fig.  5 A).	bind
40882	1	9582	7	10	NULL	0	NULL			mutation of	does not affect			D140A		alpha4beta7		structure of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_33_25652_s_232	10837471	A comparison of the staining obtained with mAbs to at least two different epitopes on the alpha4 chain (B5G10, B5E2, and HP1/2) ( 76), three different epitopes on the beta7 chain (Fib21, Fib30, and Fib504) ( 65), and an antibody that recognizes cell-surface beta7 chain only in the context of alpha4beta7 (ACT-1) ( 60,  77) showed that the binding of these mAbs was unaffected and confirmed that the D140A mutation did not grossly affect the structure of alpha4beta7 (Fig.  5 A).	bind
43255	1	9583	5	13	NULL	NULL	NULL	GP2	GP		bind					A2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_24_21443_s_197	11287414	A comparison of the structure of GP2 bound to A2 with the structure of A2I2L/V5L shows that the leucine points in the same direction as valine in molecule 1, but the side chain points away from the hydrophobic pocket (Fig.  3 A).	bind
40883	1	9583	7	NULL	NULL	0	NULL	GP2	NULL		bind	NULL				A2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_24_21443_s_197	11287414	A comparison of the structure of GP2 bound to A2 with the structure of A2I2L/V5L shows that the leucine points in the same direction as valine in molecule 1, but the side chain points away from the hydrophobic pocket (Fig.  3 A).	bind
43257	1	9584	5	13	NULL	NULL	NULL	ADP	Chemical		bind					SCS	GP	E.coli			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_16_11058_s_152	16481318	A comparison of the structure of GTP bound to pig GTP-specific SCS with the structure of ADP bound to  E. coli SCS ( ) indicates which interactions lead to specificity for the guanine base.	bind
43258	2	9584	5	13	NULL	NULL	NULL	GTP	Chemical		bind					GTP-specific SCS	GP	pig			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_16_11058_s_152	16481318	A comparison of the structure of GTP bound to pig GTP-specific SCS with the structure of ADP bound to  E. coli SCS ( ) indicates which interactions lead to specificity for the guanine base.	bind
40913	1	9584	7	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				GTP-specific SCS 	NULL	pig			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_16_11058_s_152	16481318	A comparison of the structure of GTP bound to pig GTP-specific SCS with the structure of ADP bound to  E. coli SCS ( ) indicates which interactions lead to specificity for the guanine base.	bind
40914	2	9584	7	NULL	NULL	0	NULL	ADP	NULL		bind	NULL				SCS	NULL	E.coli			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_16_11058_s_152	16481318	A comparison of the structure of GTP bound to pig GTP-specific SCS with the structure of ADP bound to  E. coli SCS ( ) indicates which interactions lead to specificity for the guanine base.	bind
43260	1	9585	5	13	NULL	NULL	NULL	Arf1	GP		bind					GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_20_0_87_s_187	15473836	A comparison of the structures  of Arf1 bound to GDP or a nonhydrolyzable analog of GTP shown in identical orientation.	bind
43261	2	9585	5	13	NULL	NULL	NULL	Arf1	GP		bind					GTP	Chemical	nonhydrolyzable analog of 			NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_20_0_87_s_187	15473836	A comparison of the structures  of Arf1 bound to GDP or a nonhydrolyzable analog of GTP shown in identical orientation.	bind
40915	1	9585	7	NULL	NULL	0	NULL	 Arf1	NULL		bind	NULL				GDP	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevcelldevbiol_20_0_87_s_187	15473836	A comparison of the structures  of Arf1 bound to GDP or a nonhydrolyzable analog of GTP shown in identical orientation.	bind
40917	2	9585	7	NULL	NULL	0	NULL	Arf1	NULL		bind	NULL				GTP	NULL	 nonhydrolyzable analog of 			NULL		0	NULL	NULL	NULL	gw70_annurevcelldevbiol_20_0_87_s_187	15473836	A comparison of the structures  of Arf1 bound to GDP or a nonhydrolyzable analog of GTP shown in identical orientation.	bind
43263	1	9586	5	13	NULL	NULL	NULL	syntaxin 1	GP		bind					Munc18-1	GP	rat			NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_1_32_s_176	12506202	A comparison of the syntaxin-bound Munc18-1 structure from rat ( ) with the syntaxin-free Munc18 structure from squid ( ) suggests that syntaxin 1 binding to Munc18-1 also does not cause a conformational change; thus, syntaxin binding generally does not induce an allosteric signal in SM proteins.	bind
43264	2	9586	5	13	NULL	NULL	NULL	statement 1	Process		does not cause					conformational change	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_1_32_s_176	12506202	A comparison of the syntaxin-bound Munc18-1 structure from rat ( ) with the syntaxin-free Munc18 structure from squid ( ) suggests that syntaxin 1 binding to Munc18-1 also does not cause a conformational change; thus, syntaxin binding generally does not induce an allosteric signal in SM proteins.	bind
43265	3	9586	5	13	NULL	NULL	NULL	statement 1	Process		does not induce					SM proteins	GP	allosteric signal			NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_1_32_s_176	12506202	A comparison of the syntaxin-bound Munc18-1 structure from rat ( ) with the syntaxin-free Munc18 structure from squid ( ) suggests that syntaxin 1 binding to Munc18-1 also does not cause a conformational change; thus, syntaxin binding generally does not induce an allosteric signal in SM proteins.	bind
40918	1	9586	7	NULL	NULL	0	NULL	syntaxin	NULL		bind	NULL				Munc18-1	NULL	rat			NULL		0	NULL	NULL	NULL	gw70_pnas_100_1_32_s_176	12506202	A comparison of the syntaxin-bound Munc18-1 structure from rat ( ) with the syntaxin-free Munc18 structure from squid ( ) suggests that syntaxin 1 binding to Munc18-1 also does not cause a conformational change; thus, syntaxin binding generally does not induce an allosteric signal in SM proteins.	bind
40920	2	9586	7	NULL	NULL	0	NULL	statement 1	NULL		does not cause	NULL				conformational change	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_100_1_32_s_176	12506202	A comparison of the syntaxin-bound Munc18-1 structure from rat ( ) with the syntaxin-free Munc18 structure from squid ( ) suggests that syntaxin 1 binding to Munc18-1 also does not cause a conformational change; thus, syntaxin binding generally does not induce an allosteric signal in SM proteins.	bind
40921	3	9586	7	NULL	NULL	0	NULL	statement 1	NULL		does not induce	NULL				SM protein	NULL	allosteric signal in			NULL		0	NULL	NULL	NULL	gw70_pnas_100_1_32_s_176	12506202	A comparison of the syntaxin-bound Munc18-1 structure from rat ( ) with the syntaxin-free Munc18 structure from squid ( ) suggests that syntaxin 1 binding to Munc18-1 also does not cause a conformational change; thus, syntaxin binding generally does not induce an allosteric signal in SM proteins.	bind
43266	1	9588	5	13	NULL	NULL	NULL	TGase 2 enzyme	GP		bind					GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_8_7180_s_317	14645372	A comparison of the TGase 2 enzyme structure recently reported bound to GDP ( ) with that of the current structures of TGase 3 indicates that although there is only a 48% sequence identity between these enzymes, there is only a 1.33  Ang  root mean square deviation relating the structures of their Calpha atoms ( Fig. 7,  A and  B).	bind
40924	1	9588	7	NULL	NULL	0	NULL	TGase 2 enzyme	NULL		bind	NULL				GDP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_7180_s_317	14645372	A comparison of the TGase 2 enzyme structure recently reported bound to GDP ( ) with that of the current structures of TGase 3 indicates that although there is only a 48% sequence identity between these enzymes, there is only a 1.33  Ang  root mean square deviation relating the structures of their Calpha atoms ( Fig. 7,  A and  B).	bind
43550	1	9589	5	13	NULL	NULL	NULL	B-FABP	GP	human	interact with			Phe104		lipid hydrocarbon tail	Chemical		double bond		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_35_27045_s_6	10854433	A comparison of the three-dimensional structures and binding properties of human B-FABP with other homologous FABPs, indicates that the binding specificity is in part the result of nonconserved amino acid Phe104, which interacts with double bonds present in the lipid hydrocarbon tail.	bind
43551	2	9589	5	13	NULL	NULL	NULL	B-FABP	GP		is a type of			Phe104		nonconserved amino acid	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_35_27045_s_6	10854433	A comparison of the three-dimensional structures and binding properties of human B-FABP with other homologous FABPs, indicates that the binding specificity is in part the result of nonconserved amino acid Phe104, which interacts with double bonds present in the lipid hydrocarbon tail.	bind
40926	1	9589	7	NULL	NULL	0	NULL	B-FABP 	NULL	human	interacts with	NULL		nonconserved amino acid Phe104		lipid hydrocarbon tail	NULL		double bond		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_35_27045_s_6	10854433	A comparison of the three-dimensional structures and binding properties of human B-FABP with other homologous FABPs, indicates that the binding specificity is in part the result of nonconserved amino acid Phe104, which interacts with double bonds present in the lipid hydrocarbon tail.	bind
56920	2	9589	7	10	NULL	0	NULL	B-FABP			is a type of			Phe104		nonconserved amino acid					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_35_27045_s_6	10854433	A comparison of the three-dimensional structures and binding properties of human B-FABP with other homologous FABPs, indicates that the binding specificity is in part the result of nonconserved amino acid Phe104, which interacts with double bonds present in the lipid hydrocarbon tail.	bind
43278	1	9590	5	13	NULL	NULL	NULL	topo VI-A' dimer	GP	structure of	is different from					DNA topoisomerase I	GP	E. coli;;structure of	DNA-binding core		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_6177_s_163	10545127	A comparison of the topo VI-A' dimer with the known structures of the DNA-binding and cleavage cores of  E.coli DNA topoisomerase I and yeast topoisomerase II shows that the overall structures are very different (Figure  5).	bind
43279	2	9590	5	13	NULL	NULL	NULL	topo VI-A' dimer	GP	structure of	is different from					DNA topoisomerase I	GP	E. coli;;structure of	cleavage core		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_6177_s_163	10545127	A comparison of the topo VI-A' dimer with the known structures of the DNA-binding and cleavage cores of  E.coli DNA topoisomerase I and yeast topoisomerase II shows that the overall structures are very different (Figure  5).	bind
43280	3	9590	5	13	NULL	NULL	NULL	topo VI-A' dimer	GP	structure of	is different from					topoisomerase II	GP	yeast;;structure of	DNA-binding core		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_6177_s_163	10545127	A comparison of the topo VI-A' dimer with the known structures of the DNA-binding and cleavage cores of  E.coli DNA topoisomerase I and yeast topoisomerase II shows that the overall structures are very different (Figure  5).	bind
43281	4	9590	5	13	NULL	NULL	NULL	topo VI-A' dimer	GP	structure of	is different from					topoisomerase II	GP	yeast;;structure of	cleavage core		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_6177_s_163	10545127	A comparison of the topo VI-A' dimer with the known structures of the DNA-binding and cleavage cores of  E.coli DNA topoisomerase I and yeast topoisomerase II shows that the overall structures are very different (Figure  5).	bind
40929	1	9590	7	10	NULL	0	NULL	topo VI-A' dimer	NULL	structure of	is different from	NULL				DNA topoisomerase I	NULL	structure of;;E.coli	DNA-binding core		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_6177_s_163	10545127	A comparison of the topo VI-A' dimer with the known structures of the DNA-binding and cleavage cores of  E.coli DNA topoisomerase I and yeast topoisomerase II shows that the overall structures are very different (Figure  5).	bind
40930	2	9590	7	10	NULL	0	NULL	topo VI-A' dimer	NULL	structure of	is different from	NULL				DNA topoisomerase I	NULL	E.coli;;structure of	cleavage core		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_6177_s_163	10545127	A comparison of the topo VI-A' dimer with the known structures of the DNA-binding and cleavage cores of  E.coli DNA topoisomerase I and yeast topoisomerase II shows that the overall structures are very different (Figure  5).	bind
47516	3	9590	7	10	NULL	0	NULL	topo VI-A' dimer	NULL	structure of	is different from	NULL				topoisomerase II	NULL	structure of;;yeast	DNA-binding core		NULL		0	NULL	NULL	NULL	gw60_embo_18_21_6177_s_163	10545127	A comparison of the topo VI-A' dimer with the known structures of the DNA-binding and cleavage cores of  E.coli DNA topoisomerase I and yeast topoisomerase II shows that the overall structures are very different (Figure  5).	bind
47517	4	9590	7	10	NULL	0	NULL	topo VI-A' dimer	NULL	structure of	is different from	NULL				topoisomerase II 	NULL	structure of;;yeast	cleavage core		NULL		0	NULL	NULL	NULL	gw60_embo_18_21_6177_s_163	10545127	A comparison of the topo VI-A' dimer with the known structures of the DNA-binding and cleavage cores of  E.coli DNA topoisomerase I and yeast topoisomerase II shows that the overall structures are very different (Figure  5).	bind
43277	1	9591	5	13	NULL	NULL	NULL	AcpS	GP		bind				3'5''-ADP CoA binding pocket				Sfp binding site		NULL		NULL	NULL	NULL	NULL	gw60_embo_19_20_5281_s_102	11032795	A comparison of the two (out of three) AcpS protomers with the two domain structures of Sfp indicates that the 3'5''-ADP CoA binding pocket of AcpS superimposes with the Sfp binding site.	bind
40933	1	9591	7	NULL	NULL	0	NULL	Sfp	NULL		bind	NULL		Sfp binding site		AcpS protomers	NULL		3'5''-ADP CoA binding pocket		NULL		NULL	NULL	NULL	NULL	gw60_embo_19_20_5281_s_102	11032795	A comparison of the two (out of three) AcpS protomers with the two domain structures of Sfp indicates that the 3'5''-ADP CoA binding pocket of AcpS superimposes with the Sfp binding site.	bind
43282	1	9592	5	13	NULL	NULL	NULL	CD46	GP		differ from		substantially	virus-binding surface		CD4	GP	human	virus-binding surface		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_11_2911_s_44	10357804	A comparison of the virus-binding surface of CD46 with those reported for human CD4 and human intercellular cell adhesion molecule-1 (ICAM-1) reveals a substantial difference in their virus recognition modes.	bind
43283	2	9592	5	13	NULL	NULL	NULL	ICAM-1	GP		is					intercellular cell adhesion molecule-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_11_2911_s_44	10357804	A comparison of the virus-binding surface of CD46 with those reported for human CD4 and human intercellular cell adhesion molecule-1 (ICAM-1) reveals a substantial difference in their virus recognition modes.	bind
43284	3	9592	5	13	NULL	NULL	NULL	CD46	GP		differ from		substantially	virus-binding surface		ICAM-1	GP	human	virus-binding surface		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_11_2911_s_44	10357804	A comparison of the virus-binding surface of CD46 with those reported for human CD4 and human intercellular cell adhesion molecule-1 (ICAM-1) reveals a substantial difference in their virus recognition modes.	bind
40997	1	9592	7	10	NULL	0	NULL	CD46	NULL		differs with	NULL		virus-binding surface		CD4	NULL	human	virus-binding surface		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_11_2911_s_44	10357804	A comparison of the virus-binding surface of CD46 with those reported for human CD4 and human intercellular cell adhesion molecule-1 (ICAM-1) reveals a substantial difference in their virus recognition modes.	bind
40998	2	9592	7	10	NULL	0	NULL	CD46	NULL		differs with	NULL		virus-binding surface		ICAM-1	NULL	human	virus-binding surface		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_11_2911_s_44	10357804	A comparison of the virus-binding surface of CD46 with those reported for human CD4 and human intercellular cell adhesion molecule-1 (ICAM-1) reveals a substantial difference in their virus recognition modes.	bind
40999	3	9592	7	NULL	NULL	0	NULL	ICAM-1	NULL		is	NULL				intercellular cell adhesion molecule-1	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_18_11_2911_s_44	10357804	A comparison of the virus-binding surface of CD46 with those reported for human CD4 and human intercellular cell adhesion molecule-1 (ICAM-1) reveals a substantial difference in their virus recognition modes.	bind
43415	1	9593	5	13	NULL	NULL	NULL	SRP54	GP		bind		high affinity			GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_89_5_703_s_72	9182758	A comparison of these results with the apparent Kd values  for GTP binding to SRP54 (2 muM) and SR  (10 muM) that were determined  by photoaffinity labeling of purified SRP and SR (Miller et al., 1993    Miller et al., 1995   ) reveals that SRP54 and SR  bind GTP  with substantially higher affinity in the context of a translocation reaction.	bind
43416	2	9593	5	13	NULL	NULL	NULL	SR	GP		bind		high affinity			GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_89_5_703_s_72	9182758	A comparison of these results with the apparent Kd values  for GTP binding to SRP54 (2 muM) and SR  (10 muM) that were determined  by photoaffinity labeling of purified SRP and SR (Miller et al., 1993    Miller et al., 1995   ) reveals that SRP54 and SR  bind GTP  with substantially higher affinity in the context of a translocation reaction.	bind
43417	3	9593	5	13	NULL	NULL	NULL	statement 1	Process		in context of					translocation reaction	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_89_5_703_s_72	9182758	A comparison of these results with the apparent Kd values  for GTP binding to SRP54 (2 muM) and SR  (10 muM) that were determined  by photoaffinity labeling of purified SRP and SR (Miller et al., 1993    Miller et al., 1995   ) reveals that SRP54 and SR  bind GTP  with substantially higher affinity in the context of a translocation reaction.	bind
43418	4	9593	5	13	NULL	NULL	NULL	statement 2	Process		in context of					translocation reaction	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_89_5_703_s_72	9182758	A comparison of these results with the apparent Kd values  for GTP binding to SRP54 (2 muM) and SR  (10 muM) that were determined  by photoaffinity labeling of purified SRP and SR (Miller et al., 1993    Miller et al., 1995   ) reveals that SRP54 and SR  bind GTP  with substantially higher affinity in the context of a translocation reaction.	bind
40934	1	9593	7	NULL	NULL	0	NULL	 GTP	NULL		bind	NULL	high affinity			SRP54	NULL	purified			NULL		NULL	NULL	NULL	NULL	gw60_cell_89_5_703_s_72	9182758	A comparison of these results with the apparent Kd values  for GTP binding to SRP54 (2 muM) and SR  (10 muM) that were determined  by photoaffinity labeling of purified SRP and SR (Miller et al., 1993    Miller et al., 1995   ) reveals that SRP54 and SR  bind GTP  with substantially higher affinity in the context of a translocation reaction.	bind
40935	2	9593	7	NULL	NULL	0	NULL	GTP	NULL		bind	NULL	high affinity			SR	NULL	purified			NULL		NULL	NULL	NULL	NULL	gw60_cell_89_5_703_s_72	9182758	A comparison of these results with the apparent Kd values  for GTP binding to SRP54 (2 muM) and SR  (10 muM) that were determined  by photoaffinity labeling of purified SRP and SR (Miller et al., 1993    Miller et al., 1995   ) reveals that SRP54 and SR  bind GTP  with substantially higher affinity in the context of a translocation reaction.	bind
40940	3	9593	7	NULL	NULL	0	NULL	statement 1	NULL		occurs in the context of	NULL				translocation reaction	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_89_5_703_s_72	9182758	A comparison of these results with the apparent Kd values  for GTP binding to SRP54 (2 muM) and SR  (10 muM) that were determined  by photoaffinity labeling of purified SRP and SR (Miller et al., 1993    Miller et al., 1995   ) reveals that SRP54 and SR  bind GTP  with substantially higher affinity in the context of a translocation reaction.	bind
40941	4	9593	7	NULL	NULL	0	NULL	statement 2	NULL		occurs in the context of	NULL				translocation reaction	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_89_5_703_s_72	9182758	A comparison of these results with the apparent Kd values  for GTP binding to SRP54 (2 muM) and SR  (10 muM) that were determined  by photoaffinity labeling of purified SRP and SR (Miller et al., 1993    Miller et al., 1995   ) reveals that SRP54 and SR  bind GTP  with substantially higher affinity in the context of a translocation reaction.	bind
43285	1	9594	5	13	NULL	NULL	NULL	HCK	GP		accommodate		easily	binding site		emodin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29618_s_130	10882732	A comparison of these structures with that of the CK2-emodin complex reveals that the binding site of HCK can easily accommodate emodin, but possibly the binding is not so tight because the entrance of the cavity is not blocked after the binding of the inhibitor.	bind
43419	2	9594	5	13	NULL	NULL	NULL	HCK	GP	cavity of 	is not blocked after					inhibitor	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29618_s_130	10882732	A comparison of these structures with that of the CK2-emodin complex reveals that the binding site of HCK can easily accommodate emodin, but possibly the binding is not so tight because the entrance of the cavity is not blocked after the binding of the inhibitor.	bind
43421	3	9594	5	13	NULL	NULL	NULL	statement 2	Process		causes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29618_s_130	10882732	A comparison of these structures with that of the CK2-emodin complex reveals that the binding site of HCK can easily accommodate emodin, but possibly the binding is not so tight because the entrance of the cavity is not blocked after the binding of the inhibitor.	bind
40944	1	9594	7	NULL	NULL	0	NULL	CK2	NULL		complex with	NULL				emodin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29618_s_130	10882732	A comparison of these structures with that of the CK2-emodin complex reveals that the binding site of HCK can easily accommodate emodin, but possibly the binding is not so tight because the entrance of the cavity is not blocked after the binding of the inhibitor.	bind
40945	2	9594	7	NULL	NULL	0	NULL	HCK	NULL		bind	NULL	may weakly			emodin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29618_s_130	10882732	A comparison of these structures with that of the CK2-emodin complex reveals that the binding site of HCK can easily accommodate emodin, but possibly the binding is not so tight because the entrance of the cavity is not blocked after the binding of the inhibitor.	bind
40949	3	9594	7	NULL	NULL	0	NULL	inhibitor	NULL	binding of	does not block	NULL				HCK	NULL		cavity of		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29618_s_130	10882732	A comparison of these structures with that of the CK2-emodin complex reveals that the binding site of HCK can easily accommodate emodin, but possibly the binding is not so tight because the entrance of the cavity is not blocked after the binding of the inhibitor.	bind
40958	4	9594	7	NULL	NULL	0	NULL	statement 2	NULL		because of	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29618_s_130	10882732	A comparison of these structures with that of the CK2-emodin complex reveals that the binding site of HCK can easily accommodate emodin, but possibly the binding is not so tight because the entrance of the cavity is not blocked after the binding of the inhibitor.	bind
43422	1	9596	5	13	NULL	NULL	NULL	Sox2	GP		bind					Oct1	GP		POUS domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_2_1449_s_253	14559893	A comparison of these two ternary complexes is of considerable interest since the separation between the Sox2 and Oct1 binding sites in the two complexes differ by three base pairs, and thus sheds light on multiple modes of interaction between Sox2 and the POUS domain of Oct1.	bind
40959	1	9596	7	NULL	NULL	0	NULL	Sox2	NULL		bind	NULL				Oct1	NULL		POUS domain		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_2_1449_s_253	14559893	A comparison of these two ternary complexes is of considerable interest since the separation between the Sox2 and Oct1 binding sites in the two complexes differ by three base pairs, and thus sheds light on multiple modes of interaction between Sox2 and the POUS domain of Oct1.	bind
43423	1	9597	5	13	NULL	NULL	NULL	thrombin receptor antibody 1809	GP		bind					WT5	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_27_16435_s_83	7608215	A comparison of thrombin receptor  antibody 1809 binding to WT5  versus  HEL cells ( 8,  24) also yielded an estimate of 5    10   receptors/cell for WT5.	bind
43424	2	9597	5	13	NULL	NULL	NULL	thrombin receptor antibody 1809	GP		bind					HEL cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_27_16435_s_83	7608215	A comparison of thrombin receptor  antibody 1809 binding to WT5  versus  HEL cells ( 8,  24) also yielded an estimate of 5    10   receptors/cell for WT5.	bind
40960	1	9597	7	NULL	NULL	0	NULL	thrombin receptor antibody 1809	NULL		bind	NULL				WT5 cells	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_27_16435_s_83	7608215	A comparison of thrombin receptor  antibody 1809 binding to WT5  versus  HEL cells ( 8,  24) also yielded an estimate of 5    10   receptors/cell for WT5.	bind
40961	2	9597	7	NULL	NULL	0	NULL	thrombin receptor antibody 1809	NULL		bind	NULL				HEL cells	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_27_16435_s_83	7608215	A comparison of thrombin receptor  antibody 1809 binding to WT5  versus  HEL cells ( 8,  24) also yielded an estimate of 5    10   receptors/cell for WT5.	bind
43427	1	9598	5	13	NULL	NULL	NULL	importin-beta	GP		wraps around			HEAT repeats		importin-alpha	GP		helical importin-beta binding domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_12_9011_s_257	10722750	A comparison of two independent structures of importin-beta ( 51) indicates that HEAT repeat domain of importin-beta is flexible, thereby permitting conformational changes that allow the tandem HEAT repeats of importin-beta to wrap around the helical importin-beta binding domain of importin-alpha ( 51).	bind
43428	2	9598	5	13	NULL	NULL	NULL	importin-beta	GP	flexibility of 	permit 			HEAT repeats		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_12_9011_s_257	10722750	A comparison of two independent structures of importin-beta ( 51) indicates that HEAT repeat domain of importin-beta is flexible, thereby permitting conformational changes that allow the tandem HEAT repeats of importin-beta to wrap around the helical importin-beta binding domain of importin-alpha ( 51).	bind
40962	1	9598	7	NULL	NULL	0	NULL	importin-beta	NULL		wrap around	NULL		tandem HEAT repeats 		importin-alpha 	NULL		helical importin-beta binding domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_12_9011_s_257	10722750	A comparison of two independent structures of importin-beta ( 51) indicates that HEAT repeat domain of importin-beta is flexible, thereby permitting conformational changes that allow the tandem HEAT repeats of importin-beta to wrap around the helical importin-beta binding domain of importin-alpha ( 51).	bind
40963	2	9598	7	NULL	NULL	0	NULL	importin-beta	NULL	flexibility of	permit	NULL		HEAT repeat domain		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_12_9011_s_257	10722750	A comparison of two independent structures of importin-beta ( 51) indicates that HEAT repeat domain of importin-beta is flexible, thereby permitting conformational changes that allow the tandem HEAT repeats of importin-beta to wrap around the helical importin-beta binding domain of importin-alpha ( 51).	bind
43429	1	9599	5	13	NULL	NULL	NULL	lck-GFP	GP		does not alter					D10	Cell	proliferation of			NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_6_809_s_49	12479826	A comparison of wild-type and transduced D10 T cells shows that lck-GFP does not alter D10 proliferation over a range of conalbumin concentrations (Supplemental Figure S1B at  http://www.immunity.	bind
40964	1	9599	7	NULL	NULL	0	NULL	lck-GFP	NULL		does not alter	NULL				D10 T cells	NULL	proliferation of			NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_6_809_s_49	12479826	A comparison of wild-type and transduced D10 T cells shows that lck-GFP does not alter D10 proliferation over a range of conalbumin concentrations (Supplemental Figure S1B at  http://www.immunity.	bind
43431	1	9600	5	13	NULL	NULL	NULL	RF-X 	GP		bind					DRA	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_nucleic-acids-res_19_6_1903200_s_10	1903200	A comparison of X box basepair positions important for RF-X binding to  DRA with sequences conserved between X boxes of other class II alpha chain  genes suggests that high affinity RF-X binding is important for a high  level of expression and may explain differences in the levels of class  II expression of different class II alpha chains.	bind
43435	2	9600	5	13	NULL	NULL	NULL	DRA	GP		is important for				X box basepair positions	statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_nucleic-acids-res_19_6_1903200_s_10	1903200	A comparison of X box basepair positions important for RF-X binding to  DRA with sequences conserved between X boxes of other class II alpha chain  genes suggests that high affinity RF-X binding is important for a high  level of expression and may explain differences in the levels of class  II expression of different class II alpha chains.	bind
40965	1	9600	7	NULL	NULL	0	NULL	RF-X	NULL		bind	NULL				DRA	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_nucleic-acids-res_19_6_1903200_s_10	1903200	A comparison of X box basepair positions important for RF-X binding to  DRA with sequences conserved between X boxes of other class II alpha chain  genes suggests that high affinity RF-X binding is important for a high  level of expression and may explain differences in the levels of class  II expression of different class II alpha chains.	bind
40967	2	9600	7	10	NULL	0	NULL	RF-X	NULL		is important for	NULL			X box basepair positions	statement 1	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_nucleic-acids-res_19_6_1903200_s_10	1903200	A comparison of X box basepair positions important for RF-X binding to  DRA with sequences conserved between X boxes of other class II alpha chain  genes suggests that high affinity RF-X binding is important for a high  level of expression and may explain differences in the levels of class  II expression of different class II alpha chains.	bind
33857	1	9801	6	11	NULL	NULL	NULL	eglin-C	GP		bind					subtilisin	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_314_2_638_s_109	14733955	A corresponding part of eglin-C bound to subtilisin [ 24] is shown in magenta.	bind
40968	1	9801	7	11	NULL	NULL	NULL	 eglin-C 	GP		bind					subtilisin	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_314_2_638_s_109	14733955	A corresponding part of eglin-C bound to subtilisin [ 24] is shown in magenta.	bind
33858	1	9802	6	11	NULL	NULL	NULL	AT4	GP		bind		specifically			Ang IV	GP				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_289_2_1075_s_223	10215690	A corresponding receptor, AT4, which specifically bound Ang IV, was thereafter identified in various tissues, including brain, heart, kidney, thymus, and adrenal from multiple species  .	bind
33859	2	9802	6	11	NULL	NULL	NULL	AT4	GP		is expressed in					brain	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_289_2_1075_s_223	10215690	A corresponding receptor, AT4, which specifically bound Ang IV, was thereafter identified in various tissues, including brain, heart, kidney, thymus, and adrenal from multiple species  .	bind
33860	3	9802	6	11	NULL	NULL	NULL	AT4	GP		is expressed in					kidney	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_289_2_1075_s_223	10215690	A corresponding receptor, AT4, which specifically bound Ang IV, was thereafter identified in various tissues, including brain, heart, kidney, thymus, and adrenal from multiple species  .	bind
33861	4	9802	6	11	NULL	NULL	NULL	AT4	GP		is expressed in					heart	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_289_2_1075_s_223	10215690	A corresponding receptor, AT4, which specifically bound Ang IV, was thereafter identified in various tissues, including brain, heart, kidney, thymus, and adrenal from multiple species  .	bind
33862	5	9802	6	11	NULL	NULL	NULL	AT4	GP		is expressed in					thymus	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_289_2_1075_s_223	10215690	A corresponding receptor, AT4, which specifically bound Ang IV, was thereafter identified in various tissues, including brain, heart, kidney, thymus, and adrenal from multiple species  .	bind
33863	6	9802	6	11	NULL	NULL	NULL	AT4	GP		is expressed in					adrenal	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_289_2_1075_s_223	10215690	A corresponding receptor, AT4, which specifically bound Ang IV, was thereafter identified in various tissues, including brain, heart, kidney, thymus, and adrenal from multiple species  .	bind
48890	7	9802	6	11	NULL	NULL	NULL	AT4	GP		is a type of					receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_289_2_1075_s_223	10215690	A corresponding receptor, AT4, which specifically bound Ang IV, was thereafter identified in various tissues, including brain, heart, kidney, thymus, and adrenal from multiple species  .	bind
40969	1	9802	7	11	NULL	NULL	NULL	AT4 receptor	GP		bind		specifically			Ang IV	GP				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_289_2_1075_s_223	10215690	A corresponding receptor, AT4, which specifically bound Ang IV, was thereafter identified in various tissues, including brain, heart, kidney, thymus, and adrenal from multiple species  .	bind
48891	2	9802	7	11	NULL	NULL	NULL	AT4 receptor	GP		is expressed in					brain	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_289_2_1075_s_223	10215690	A corresponding receptor, AT4, which specifically bound Ang IV, was thereafter identified in various tissues, including brain, heart, kidney, thymus, and adrenal from multiple species  .	bind
48893	3	9802	7	11	NULL	NULL	NULL	AT4 receptor	GP		is expressed in					heart	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_289_2_1075_s_223	10215690	A corresponding receptor, AT4, which specifically bound Ang IV, was thereafter identified in various tissues, including brain, heart, kidney, thymus, and adrenal from multiple species  .	bind
48894	4	9802	7	11	NULL	NULL	NULL	AT4 receptor	GP		is expressed in					kidney	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_289_2_1075_s_223	10215690	A corresponding receptor, AT4, which specifically bound Ang IV, was thereafter identified in various tissues, including brain, heart, kidney, thymus, and adrenal from multiple species  .	bind
48895	5	9802	7	11	NULL	NULL	NULL	AT4 receptor	GP		is expressed in					thymus	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_289_2_1075_s_223	10215690	A corresponding receptor, AT4, which specifically bound Ang IV, was thereafter identified in various tissues, including brain, heart, kidney, thymus, and adrenal from multiple species  .	bind
48896	6	9802	7	11	NULL	NULL	NULL	AT4 receptor	GP		is expressed in					adrenal	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_289_2_1075_s_223	10215690	A corresponding receptor, AT4, which specifically bound Ang IV, was thereafter identified in various tissues, including brain, heart, kidney, thymus, and adrenal from multiple species  .	bind
33864	1	9803	6	11	NULL	NULL	NULL	accessory factor	GP		bind					gAF2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_43_39885_s_124	11518712	A corresponding segment with a block mutation that prevents accessory factor binding to gAF2 does not promote complex formation ( open triangles).	bind
48897	2	9803	6	11	NULL	NULL	NULL	block mutation	Process		prevents					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_43_39885_s_124	11518712	A corresponding segment with a block mutation that prevents accessory factor binding to gAF2 does not promote complex formation ( open triangles).	bind
48898	3	9803	6	11	NULL	NULL	NULL	statement 2	Process		does not promote					complex	GP	formation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_43_39885_s_124	11518712	A corresponding segment with a block mutation that prevents accessory factor binding to gAF2 does not promote complex formation ( open triangles).	bind
40970	1	9803	7	11	NULL	NULL	NULL	accessory factor 	GP		bind					gAF2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_43_39885_s_124	11518712	A corresponding segment with a block mutation that prevents accessory factor binding to gAF2 does not promote complex formation ( open triangles).	bind
40971	2	9803	7	11	NULL	NULL	NULL	block mutation	Process		prevents					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_43_39885_s_124	11518712	A corresponding segment with a block mutation that prevents accessory factor binding to gAF2 does not promote complex formation ( open triangles).	bind
40972	3	9803	7	11	NULL	NULL	NULL	statement 2	Process		does not promote					complex	GP	formation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_43_39885_s_124	11518712	A corresponding segment with a block mutation that prevents accessory factor binding to gAF2 does not promote complex formation ( open triangles).	bind
33866	1	9805	6	11	NULL	NULL	NULL	ATP	Chemical		bind					type IIA topoisomerases	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_187_24_8531_s_11	16321962	A coumarin, novobiocin, competitively inhibits ATP binding to type IIA topoisomerases ( ).	bind
33867	2	9805	6	11	NULL	NULL	NULL	novobiocin	Chemical		is a type of					coumarin	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_187_24_8531_s_11	16321962	A coumarin, novobiocin, competitively inhibits ATP binding to type IIA topoisomerases ( ).	bind
33868	3	9805	6	11	NULL	NULL	NULL	novobiocin	Chemical		inhibits		competitively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_187_24_8531_s_11	16321962	A coumarin, novobiocin, competitively inhibits ATP binding to type IIA topoisomerases ( ).	bind
40974	1	9805	7	11	NULL	NULL	NULL	ATP	Chemical		bind					type IIA topoisomerases	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_187_24_8531_s_11	16321962	A coumarin, novobiocin, competitively inhibits ATP binding to type IIA topoisomerases ( ).	bind
40975	2	9805	7	11	NULL	NULL	NULL	novobiocin	Chemical		is a type of					coumarin	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_187_24_8531_s_11	16321962	A coumarin, novobiocin, competitively inhibits ATP binding to type IIA topoisomerases ( ).	bind
40976	3	9805	7	11	NULL	NULL	NULL	novobiocin	Chemical		inhibits		competitively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_187_24_8531_s_11	16321962	A coumarin, novobiocin, competitively inhibits ATP binding to type IIA topoisomerases ( ).	bind
33869	1	9807	6	11	NULL	NULL	NULL	RyR2	GP		bind					FKBP12.6	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_45_37941_s_174	16157601	A CPVT-linked RyR2 mutant in the central region (S2246L) also displays normal RyR2-FKBP12.6 binding ( ).	bind
33870	2	9807	6	11	NULL	NULL	NULL	RyR2	GP	mutant	bind			S2246L		FKBP12.6	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_45_37941_s_174	16157601	A CPVT-linked RyR2 mutant in the central region (S2246L) also displays normal RyR2-FKBP12.6 binding ( ).	bind
40978	1	9807	7	11	NULL	NULL	NULL	CPVT-linked RyR2 	GP	mutant	bind		normally	central region S2246L		FKBP12.6	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_45_37941_s_174	16157601	A CPVT-linked RyR2 mutant in the central region (S2246L) also displays normal RyR2-FKBP12.6 binding ( ).	bind
33871	1	9808	6	11	NULL	NULL	NULL	Brk	GP		represses					D-h	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_development_131_11_2681_s_305	15128656	A CRE in the D- h repression element is required for repression   Given the genetic evidence that Brk represses D- h expression and that Brk binds the CMB element in vitro, the most straightforward hypothesis is that Brk acts directly through the CMB in vivo to repress D- h expression.	bind
33872	2	9808	6	11	NULL	NULL	NULL	Brk	GP		bind									CMB element	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_development_131_11_2681_s_305	15128656	A CRE in the D- h repression element is required for repression   Given the genetic evidence that Brk represses D- h expression and that Brk binds the CMB element in vitro, the most straightforward hypothesis is that Brk acts directly through the CMB in vivo to repress D- h expression.	bind
33873	3	9808	6	11	NULL	NULL	NULL	Brk	GP		acts through		directly							CMB	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_development_131_11_2681_s_305	15128656	A CRE in the D- h repression element is required for repression   Given the genetic evidence that Brk represses D- h expression and that Brk binds the CMB element in vitro, the most straightforward hypothesis is that Brk acts directly through the CMB in vivo to repress D- h expression.	bind
33874	4	9808	6	11	NULL	NULL	NULL	statement 3	Process		leads to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_131_11_2681_s_305	15128656	A CRE in the D- h repression element is required for repression   Given the genetic evidence that Brk represses D- h expression and that Brk binds the CMB element in vitro, the most straightforward hypothesis is that Brk acts directly through the CMB in vivo to repress D- h expression.	bind
40979	1	9808	7	11	NULL	NULL	NULL	Brk	GP		binds									CMB element	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_development_131_11_2681_s_305	15128656	A CRE in the D- h repression element is required for repression   Given the genetic evidence that Brk represses D- h expression and that Brk binds the CMB element in vitro, the most straightforward hypothesis is that Brk acts directly through the CMB in vivo to repress D- h expression.	bind
40980	2	9808	7	11	NULL	NULL	NULL	Brk	GP		acts through		directly							CMB	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_development_131_11_2681_s_305	15128656	A CRE in the D- h repression element is required for repression   Given the genetic evidence that Brk represses D- h expression and that Brk binds the CMB element in vitro, the most straightforward hypothesis is that Brk acts directly through the CMB in vivo to repress D- h expression.	bind
40981	3	9808	7	11	NULL	NULL	NULL	Brk	GP		repress					D- h	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_development_131_11_2681_s_305	15128656	A CRE in the D- h repression element is required for repression   Given the genetic evidence that Brk represses D- h expression and that Brk binds the CMB element in vitro, the most straightforward hypothesis is that Brk acts directly through the CMB in vivo to repress D- h expression.	bind
40982	4	9808	7	11	NULL	NULL	NULL	statement 3	Process		occur through					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_131_11_2681_s_305	15128656	A CRE in the D- h repression element is required for repression   Given the genetic evidence that Brk represses D- h expression and that Brk binds the CMB element in vitro, the most straightforward hypothesis is that Brk acts directly through the CMB in vivo to repress D- h expression.	bind
33875	1	9809	6	11	NULL	NULL	NULL	statement 3	Process		bind					CREB1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5329_s_30	15964791	A CRE-like element in the 5''-flanking region of the MuSK gene binds to CREB1 to inhibit the MuSK promoter activity.	bind
33876	2	9809	6	11	NULL	NULL	NULL	statement 1	Process		inhibits					MuSK	GP	activity of 		promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5329_s_30	15964791	A CRE-like element in the 5''-flanking region of the MuSK gene binds to CREB1 to inhibit the MuSK promoter activity.	bind
56787	3	9809	6	11	NULL	NULL	NULL				is present in				CRE element	MuSK gene	GP			5''-flanking region	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5329_s_30	15964791	A CRE-like element in the 5''-flanking region of the MuSK gene binds to CREB1 to inhibit the MuSK promoter activity.	bind
40984	1	9809	7	11	NULL	NULL	NULL	 CREB1	GP		binds					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5329_s_30	15964791	A CRE-like element in the 5''-flanking region of the MuSK gene binds to CREB1 to inhibit the MuSK promoter activity.	bind
40985	2	9809	7	11	NULL	NULL	NULL	statement 1	Process		inhibit					MuSK	GP	activity of		promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5329_s_30	15964791	A CRE-like element in the 5''-flanking region of the MuSK gene binds to CREB1 to inhibit the MuSK promoter activity.	bind
56788	3	9809	7	11	NULL	NULL	NULL				is present in				CRE element	MuSK gene	GP			5''-flanking region	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5329_s_30	15964791	A CRE-like element in the 5''-flanking region of the MuSK gene binds to CREB1 to inhibit the MuSK promoter activity.	bind
33945	1	9810	6	11	NULL	NULL	NULL	CREB	GP		bind			B-ZIP domain		oligonucleotide	NucleicAcid			CRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_967_s_149	9447994	A CREB B-ZIP homodimer retarded the mobility of the radiolabeled double-stranded 25-bp oligonucleotide probe containing a single consensus CRE (Fig.  3A, lane 2), and an equimolar concentration of A-CREB (lane 3) effectively inhibited binding of the CREB B-ZIP domain to the CRE-containing oligonucleotide.	bind
33946	2	9810	6	11	NULL	NULL	NULL	A-CREB	GP		inhibits		effectively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_967_s_149	9447994	A CREB B-ZIP homodimer retarded the mobility of the radiolabeled double-stranded 25-bp oligonucleotide probe containing a single consensus CRE (Fig.  3A, lane 2), and an equimolar concentration of A-CREB (lane 3) effectively inhibited binding of the CREB B-ZIP domain to the CRE-containing oligonucleotide.	bind
40986	1	9810	7	11	NULL	NULL	NULL	CREB	GP		bind			B-ZIP domain		oligonucleotide	NucleicAcid			CRE	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_967_s_149	9447994	A CREB B-ZIP homodimer retarded the mobility of the radiolabeled double-stranded 25-bp oligonucleotide probe containing a single consensus CRE (Fig.  3A, lane 2), and an equimolar concentration of A-CREB (lane 3) effectively inhibited binding of the CREB B-ZIP domain to the CRE-containing oligonucleotide.	bind
40987	2	9810	7	11	NULL	NULL	NULL	A-CREB 	GP		inhibits		effectively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_2_967_s_149	9447994	A CREB B-ZIP homodimer retarded the mobility of the radiolabeled double-stranded 25-bp oligonucleotide probe containing a single consensus CRE (Fig.  3A, lane 2), and an equimolar concentration of A-CREB (lane 3) effectively inhibited binding of the CREB B-ZIP domain to the CRE-containing oligonucleotide.	bind
33877	1	9811	6	11	NULL	NULL	NULL	CREB Family Member	GP		bind					BDNF	GP			CRE	NULL		NULL	NULL	NULL	NULL	gw60_neuron_20_4_709_s_282	9581763	A CREB Family Member Binds to the  BDNF-CRE and Mediates  BDNF Transcription	bind
33878	2	9811	6	11	NULL	NULL	NULL	statement 1	Process		mediates					BDNF	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw60_neuron_20_4_709_s_282	9581763	A CREB Family Member Binds to the  BDNF-CRE and Mediates  BDNF Transcription	bind
40988	1	9811	7	11	NULL	NULL	NULL	CREB Family Member 	GP		binds to					BDNF	GP			CRE	NULL		NULL	NULL	NULL	NULL	gw60_neuron_20_4_709_s_282	9581763	A CREB Family Member Binds to the  BDNF-CRE and Mediates  BDNF Transcription	bind
40989	2	9811	7	11	NULL	NULL	NULL	statement 1	Process		mediates					BDNF	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw60_neuron_20_4_709_s_282	9581763	A CREB Family Member Binds to the  BDNF-CRE and Mediates  BDNF Transcription	bind
33879	1	9812	6	11	NULL	NULL	NULL	Ren-1c	GP		contains				enhancer					CREB/cAMP-response element modulator protein binding site	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_35_32489_s_251	11432851	A CREB/cAMP-response element modulator protein binding site within the  Ren-1c enhancer located at  2.6 kb is critical for the enhancer function.	bind
33880	2	9812	6	11	NULL	NULL	NULL	Ren-1c	GP		is critical for				CREB/cAMP-response element modulator protein binding site	Ren-1c	GP	function of 		enhancer	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_35_32489_s_251	11432851	A CREB/cAMP-response element modulator protein binding site within the  Ren-1c enhancer located at  2.6 kb is critical for the enhancer function.	bind
40990	1	9812	7	11	NULL	NULL	NULL	Ren-1c	GP		contains				enhancer					CREB/cAMP-response element modulator protein binding site 	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_35_32489_s_251	11432851	A CREB/cAMP-response element modulator protein binding site within the  Ren-1c enhancer located at  2.6 kb is critical for the enhancer function.	bind
40991	2	9812	7	11	NULL	NULL	NULL	Ren-1c	GP		is critical for				CREB/cAMP-response element modulator protein binding site 	Ren-1c	GP	function of		enhancer	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_35_32489_s_251	11432851	A CREB/cAMP-response element modulator protein binding site within the  Ren-1c enhancer located at  2.6 kb is critical for the enhancer function.	bind
33881	1	9813	6	11	NULL	NULL	NULL	CREB/CREM family protein	GP		bind					A3 AR	GP	partial;;mouse		CRE site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_62_5_1167_s_211	12391281	A CREB/CREM family protein binds the partial CRE of the mouse A3 AR promoter.	bind
40992	1	9813	7	11	NULL	NULL	NULL	CREB/CREM family protein	GP		bind					A3 AR	GP	partial;;mouse		CRE site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_62_5_1167_s_211	12391281	A CREB/CREM family protein binds the partial CRE of the mouse A3 AR promoter.	bind
34721	1	9815	6	11	NULL	NULL	NULL	Abl	GP		bind			SH3 domain					proline in the SH2-CD linker		NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_27_s_174	12887890	A critical component of the c-Abl regulatory mechanism is shared with Src kinases: the Abl SH3 domain binds to a single proline (Pro242 in type Ib/IV c-Abl) in the SH2-CD linker that is conserved in Src family members.	bind
34972	2	9815	6	11	NULL	NULL	NULL				is conserved in			SH2-CD linker		Src family members	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_27_s_174	12887890	A critical component of the c-Abl regulatory mechanism is shared with Src kinases: the Abl SH3 domain binds to a single proline (Pro242 in type Ib/IV c-Abl) in the SH2-CD linker that is conserved in Src family members.	bind
40995	1	9815	7	11	NULL	NULL	NULL	Abl	GP		binds to			SH3 domain					Proline in SH2-CD linker		NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_27_s_174	12887890	A critical component of the c-Abl regulatory mechanism is shared with Src kinases: the Abl SH3 domain binds to a single proline (Pro242 in type Ib/IV c-Abl) in the SH2-CD linker that is conserved in Src family members.	bind
40996	2	9815	7	11	NULL	NULL	NULL				is conserved in			SH2-CD linker		Src family members	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_27_s_174	12887890	A critical component of the c-Abl regulatory mechanism is shared with Src kinases: the Abl SH3 domain binds to a single proline (Pro242 in type Ib/IV c-Abl) in the SH2-CD linker that is conserved in Src family members.	bind
34064	1	9816	6	11	NULL	NULL	NULL	SecA	GP		bind					chaperone-precursor complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_66_0_199_s_212	9242906	A critical cytoplasmic component of the  translocase is SecA, which binds to the chaperone-precursor complex and to SecY,  dependent on the presence of anionic phospholipids in the membrane ( 98).	bind
34066	2	9816	6	11	NULL	NULL	NULL	SecA	GP		bind					SecY	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_66_0_199_s_212	9242906	A critical cytoplasmic component of the  translocase is SecA, which binds to the chaperone-precursor complex and to SecY,  dependent on the presence of anionic phospholipids in the membrane ( 98).	bind
34718	3	9816	6	11	NULL	NULL	NULL	statement 1	Process		is dependent on					anionic phospholipids	Chemical	presence of			NULL	membrane	NULL	NULL	NULL	NULL	gw70_annurevbiochem_66_0_199_s_212	9242906	A critical cytoplasmic component of the  translocase is SecA, which binds to the chaperone-precursor complex and to SecY,  dependent on the presence of anionic phospholipids in the membrane ( 98).	bind
34719	4	9816	6	11	NULL	NULL	NULL	statement 2	Process		is dependent on					anionic phospholipids	Chemical	presence of			NULL	membrane	NULL	NULL	NULL	NULL	gw70_annurevbiochem_66_0_199_s_212	9242906	A critical cytoplasmic component of the  translocase is SecA, which binds to the chaperone-precursor complex and to SecY,  dependent on the presence of anionic phospholipids in the membrane ( 98).	bind
34720	5	9816	6	11	NULL	NULL	NULL	SecA	GP		is a critical cytoplasmic component of					translocase	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_66_0_199_s_212	9242906	A critical cytoplasmic component of the  translocase is SecA, which binds to the chaperone-precursor complex and to SecY,  dependent on the presence of anionic phospholipids in the membrane ( 98).	bind
41055	1	9816	7	11	NULL	NULL	NULL	SecA	GP		is a critical cytoplasmic component of					translocase 	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_66_0_199_s_212	9242906	A critical cytoplasmic component of the  translocase is SecA, which binds to the chaperone-precursor complex and to SecY,  dependent on the presence of anionic phospholipids in the membrane ( 98).	bind
41056	2	9816	7	11	NULL	NULL	NULL	chaperone	GP		complex with					precursor	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_66_0_199_s_212	9242906	A critical cytoplasmic component of the  translocase is SecA, which binds to the chaperone-precursor complex and to SecY,  dependent on the presence of anionic phospholipids in the membrane ( 98).	bind
41057	3	9816	7	11	NULL	NULL	NULL	SecA	GP		binds to					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_66_0_199_s_212	9242906	A critical cytoplasmic component of the  translocase is SecA, which binds to the chaperone-precursor complex and to SecY,  dependent on the presence of anionic phospholipids in the membrane ( 98).	bind
41058	4	9816	7	11	NULL	NULL	NULL	SecA	GP		binds to					SecY	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_66_0_199_s_212	9242906	A critical cytoplasmic component of the  translocase is SecA, which binds to the chaperone-precursor complex and to SecY,  dependent on the presence of anionic phospholipids in the membrane ( 98).	bind
41059	5	9816	7	11	NULL	NULL	NULL	statement 3	Process		depends on					anionic phospholipids	Chemical				NULL	in the membrane	NULL	NULL	NULL	NULL	gw70_annurevbiochem_66_0_199_s_212	9242906	A critical cytoplasmic component of the  translocase is SecA, which binds to the chaperone-precursor complex and to SecY,  dependent on the presence of anionic phospholipids in the membrane ( 98).	bind
41060	6	9816	7	11	NULL	NULL	NULL	statement 4	Process		depends on					anionic phospholipids	Chemical				NULL	in the membrane	NULL	NULL	NULL	NULL	gw70_annurevbiochem_66_0_199_s_212	9242906	A critical cytoplasmic component of the  translocase is SecA, which binds to the chaperone-precursor complex and to SecY,  dependent on the presence of anionic phospholipids in the membrane ( 98).	bind
34068	1	9817	6	11	NULL	NULL	NULL	DnaA protein	GP	Escherichia coli	bind		cooperatively			Plasmid RK2	NucleicAcid			Replication Origin	NULL		NULL	NULL	NULL	NULL	gw60_embo_17_15_4511_s_752	9687517	A Critical DnaA Box Directs the Cooperative Binding of the Escherichia coli DnaA Protein to the Plasmid RK2 Replication Origin.	bind
34069	2	9817	6	11	NULL	NULL	NULL				directs				DnaA Box	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_15_4511_s_752	9687517	A Critical DnaA Box Directs the Cooperative Binding of the Escherichia coli DnaA Protein to the Plasmid RK2 Replication Origin.	bind
41061	1	9817	7	11	NULL	NULL	NULL	DnaA Protein	GP	 Escherichia coli	bind		cooperatively			Plasmid RK2	NucleicAcid			Replication Origin	NULL		NULL	NULL	NULL	NULL	gw60_embo_17_15_4511_s_752	9687517	A Critical DnaA Box Directs the Cooperative Binding of the Escherichia coli DnaA Protein to the Plasmid RK2 Replication Origin.	bind
41062	2	9817	7	11	NULL	NULL	NULL				directs				DnaA Box	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_15_4511_s_752	9687517	A Critical DnaA Box Directs the Cooperative Binding of the Escherichia coli DnaA Protein to the Plasmid RK2 Replication Origin.	bind
34071	1	9819	6	11	NULL	NULL	NULL	IL-4	GP		bind					IL-4R	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_9_1_13_s_14	9697832	A critical event in the activation of IL-4 responsive genes involves the phosphorylation and nuclear translocation of the signal transducer and activator of transcription Stat6, which is specifically activated by binding of IL-4 to the IL-4R (  Hou et al. 1994  ; Ryan et al. 1996  ).	bind
34072	2	9819	6	11	NULL	NULL	NULL	Stat	GP		is					signal transducer and activator of transcription	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_9_1_13_s_14	9697832	A critical event in the activation of IL-4 responsive genes involves the phosphorylation and nuclear translocation of the signal transducer and activator of transcription Stat6, which is specifically activated by binding of IL-4 to the IL-4R (  Hou et al. 1994  ; Ryan et al. 1996  ).	bind
34074	3	9819	6	11	NULL	NULL	NULL	IL-4 responsive genes	GP	activation of	involves					Stat6	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_immunity_9_1_13_s_14	9697832	A critical event in the activation of IL-4 responsive genes involves the phosphorylation and nuclear translocation of the signal transducer and activator of transcription Stat6, which is specifically activated by binding of IL-4 to the IL-4R (  Hou et al. 1994  ; Ryan et al. 1996  ).	bind
34075	4	9819	6	11	NULL	NULL	NULL	IL-4 responsive genes	GP	activation of	involves					Stat6	GP	nuclear translocation of 			NULL		NULL	NULL	NULL	NULL	gw60_immunity_9_1_13_s_14	9697832	A critical event in the activation of IL-4 responsive genes involves the phosphorylation and nuclear translocation of the signal transducer and activator of transcription Stat6, which is specifically activated by binding of IL-4 to the IL-4R (  Hou et al. 1994  ; Ryan et al. 1996  ).	bind
34077	5	9819	6	11	NULL	NULL	NULL	statement 1	Process		activates					Stat6	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_9_1_13_s_14	9697832	A critical event in the activation of IL-4 responsive genes involves the phosphorylation and nuclear translocation of the signal transducer and activator of transcription Stat6, which is specifically activated by binding of IL-4 to the IL-4R (  Hou et al. 1994  ; Ryan et al. 1996  ).	bind
41063	1	9819	7	11	NULL	NULL	NULL	IL-4 responsive genes	GP	activation of 	involves					Stat6	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_immunity_9_1_13_s_14	9697832	A critical event in the activation of IL-4 responsive genes involves the phosphorylation and nuclear translocation of the signal transducer and activator of transcription Stat6, which is specifically activated by binding of IL-4 to the IL-4R (  Hou et al. 1994  ; Ryan et al. 1996  ).	bind
41064	2	9819	7	11	NULL	NULL	NULL	IL-4 responsive genes	GP	activation of	involves					Stat6	GP	nuclear translocation of			NULL		NULL	NULL	NULL	NULL	gw60_immunity_9_1_13_s_14	9697832	A critical event in the activation of IL-4 responsive genes involves the phosphorylation and nuclear translocation of the signal transducer and activator of transcription Stat6, which is specifically activated by binding of IL-4 to the IL-4R (  Hou et al. 1994  ; Ryan et al. 1996  ).	bind
41068	3	9819	7	11	NULL	NULL	NULL	IL-4	GP		bind					IL-4R	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_9_1_13_s_14	9697832	A critical event in the activation of IL-4 responsive genes involves the phosphorylation and nuclear translocation of the signal transducer and activator of transcription Stat6, which is specifically activated by binding of IL-4 to the IL-4R (  Hou et al. 1994  ; Ryan et al. 1996  ).	bind
41077	4	9819	7	11	NULL	NULL	NULL	statement 3	Process		activates		specifically			Stat6	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_9_1_13_s_14	9697832	A critical event in the activation of IL-4 responsive genes involves the phosphorylation and nuclear translocation of the signal transducer and activator of transcription Stat6, which is specifically activated by binding of IL-4 to the IL-4R (  Hou et al. 1994  ; Ryan et al. 1996  ).	bind
41080	5	9819	7	11	NULL	NULL	NULL	Stat6	GP		is					signal transducer and activator of transcription 6	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_9_1_13_s_14	9697832	A critical event in the activation of IL-4 responsive genes involves the phosphorylation and nuclear translocation of the signal transducer and activator of transcription Stat6, which is specifically activated by binding of IL-4 to the IL-4R (  Hou et al. 1994  ; Ryan et al. 1996  ).	bind
49560	1	9820	6	11	NULL	NULL	NULL	dATP	Chemical		bind					CTX II	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17869_s_199	10364232	A critical examination of the observed intramolecular NOEs between the sugar and the adenine ring (in the dATP molecule bound to CTX II) shows that intramolecular NOEs (between H8 proton of the adenine ring and the H1'', H2'', H2''', H4'' of the deoxy ribose sugar) are quite similar to that expected for the  anti conformation (of the nucleotide).	bind
49547	1	9820	7	11	NULL	NULL	NULL	dATP molecule	Chemical		bind					CTXII	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_17869_s_199	10364232	A critical examination of the observed intramolecular NOEs between the sugar and the adenine ring (in the dATP molecule bound to CTX II) shows that intramolecular NOEs (between H8 proton of the adenine ring and the H1'', H2'', H2''', H4'' of the deoxy ribose sugar) are quite similar to that expected for the  anti conformation (of the nucleotide).	bind
34080	1	9822	6	11	NULL	NULL	NULL	TR	GP		bind					TH-inducible genes	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_50_41222_s_35	16236718	A critical parameter for the dual function model is TR binding to TH-inducible genes  in vivo.	bind
41094	1	9822	7	11	NULL	NULL	NULL	TR	GP		bind					TH-inducible genes	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_50_41222_s_35	16236718	A critical parameter for the dual function model is TR binding to TH-inducible genes  in vivo.	bind
34084	1	9823	6	11	NULL	NULL	NULL	Crm1	GP		bind					target proteins	GP		leucine-rich NES sequences		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7273_s_159	10982844	A critical regulatory event in nucleocytoplasmic transport is the binding of a nuclear export receptor such as Crm1 to the leucine-rich NES sequences of target proteins.	bind
34086	2	9823	6	11	NULL	NULL	NULL	Crm1	GP		is a type of					nuclear export receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7273_s_159	10982844	A critical regulatory event in nucleocytoplasmic transport is the binding of a nuclear export receptor such as Crm1 to the leucine-rich NES sequences of target proteins.	bind
34088	3	9823	6	11	NULL	NULL	NULL	statement 1	Process		is a regulatory event in		critical			nucleocytoplasmic transport	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7273_s_159	10982844	A critical regulatory event in nucleocytoplasmic transport is the binding of a nuclear export receptor such as Crm1 to the leucine-rich NES sequences of target proteins.	bind
41099	1	9823	7	11	NULL	NULL	NULL	Crm1	GP		bind					target proteins	GP		leucine-rich NES sequences 		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7273_s_159	10982844	A critical regulatory event in nucleocytoplasmic transport is the binding of a nuclear export receptor such as Crm1 to the leucine-rich NES sequences of target proteins.	bind
41101	2	9823	7	11	NULL	NULL	NULL	Crm1	GP		is a type of					nuclear export receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7273_s_159	10982844	A critical regulatory event in nucleocytoplasmic transport is the binding of a nuclear export receptor such as Crm1 to the leucine-rich NES sequences of target proteins.	bind
41120	3	9823	7	11	NULL	NULL	NULL	statement 1	Process		regulates					nucleocytoplasmic transport	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7273_s_159	10982844	A critical regulatory event in nucleocytoplasmic transport is the binding of a nuclear export receptor such as Crm1 to the leucine-rich NES sequences of target proteins.	bind
34089	1	9824	6	11	NULL	NULL	NULL	PP1	GP		bind			threonine 340		c-SrcP	GP	mouse	ATP-binding pocket		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_1_59_s_175	16267045	A critical residue for PP1 to fit into the ATP binding pocket of mouse c-SrcP is threonine 340 (corresponding to v-Src threonine 338).	bind
41123	1	9824	7	11	NULL	NULL	NULL	PP1	GP		fits into the			threonine 340		c-SrcP	GP	mouse	ATP binding pocket		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_1_59_s_175	16267045	A critical residue for PP1 to fit into the ATP binding pocket of mouse c-SrcP is threonine 340 (corresponding to v-Src threonine 338).	bind
41129	2	9824	7	11	NULL	NULL	NULL	c-SrcP	GP		corresponds to			threonine 340 		v-Src 	GP		threonine 338		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_1_59_s_175	16267045	A critical residue for PP1 to fit into the ATP binding pocket of mouse c-SrcP is threonine 340 (corresponding to v-Src threonine 338).	bind
34090	1	9825	6	11	NULL	NULL	NULL	VWF	GP		bind					glycoprotein Ib-IX	GP	platelet			NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_blood_106_6_15941906_s_1	15941906	A critical role for 14-3-3zeta protein in regulating the VWF binding function of platelet glycoprotein Ib-IX and its therapeutic implications..	bind
34091	2	9825	6	11	NULL	NULL	NULL	14-3-3 zeta protein	GP		regulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_blood_106_6_15941906_s_1	15941906	A critical role for 14-3-3zeta protein in regulating the VWF binding function of platelet glycoprotein Ib-IX and its therapeutic implications..	bind
41140	1	9825	7	11	NULL	NULL	NULL	VWF	GP		bind					glycoprotein Ib-IX	GP	platelet			NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_blood_106_6_15941906_s_1	15941906	A critical role for 14-3-3zeta protein in regulating the VWF binding function of platelet glycoprotein Ib-IX and its therapeutic implications..	bind
41141	2	9825	7	11	NULL	NULL	NULL	14-3-3zeta protein	GP		regulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_blood_106_6_15941906_s_1	15941906	A critical role for 14-3-3zeta protein in regulating the VWF binding function of platelet glycoprotein Ib-IX and its therapeutic implications..	bind
34157	1	9826	6	11	NULL	NULL	NULL	Cbl	GP		bind			phosphotyrosine-binding domain		Syk	GP		phosphotyrosine 323		NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_20_0_669_s_1334	11861615	A critical role for Cbl phosphotyrosine-binding domain binding to Syk phosphotyrosine  323.	bind
41142	1	9826	7	11	NULL	NULL	NULL	Cbl	GP		bind			phosphotyrosine-binding domain		Syk	GP		phosphotyrosine 323		NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_20_0_669_s_1334	11861615	A critical role for Cbl phosphotyrosine-binding domain binding to Syk phosphotyrosine  323.	bind
34158	1	9829	6	11	NULL	NULL	NULL	TAT protein	GP		bind									TAR element	NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_retrovirology_2_1_16293193_s_3	16293193	A critical step in the production of new HIV virions involves  the TAT protein binding to the TAR element.	bind
34159	2	9829	6	11	NULL	NULL	NULL	HIV virions	Organism	production of	involves					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_retrovirology_2_1_16293193_s_3	16293193	A critical step in the production of new HIV virions involves  the TAT protein binding to the TAR element.	bind
41143	1	9829	7	11	NULL	NULL	NULL	TAT protein	GP		bind									TAR element	NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_retrovirology_2_1_16293193_s_3	16293193	A critical step in the production of new HIV virions involves  the TAT protein binding to the TAR element.	bind
41144	2	9829	7	11	NULL	NULL	NULL	new HIV virions	Organism	production of	involves					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_retrovirology_2_1_16293193_s_3	16293193	A critical step in the production of new HIV virions involves  the TAT protein binding to the TAR element.	bind
34160	1	9830	6	11	NULL	NULL	NULL	METS	GP		bind		selectively			c-Myc	GP			Ets site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_cell_109_2_169_s_255	12007404	A critical test of the ability of METS to discriminate between monomeric sites in cell cycle-regulatory genes and composite elements in cell type-specific genes was provided by ChIP assays, which clearly established selective binding of METS to Ets sites in the  c-Myc,  Cdc2, and  p54 promoters, but not to the composite AP-1/Ets site in the  SR-A promoter in terminally differentiated macrophages.	bind
34161	2	9830	6	11	NULL	NULL	NULL	METS	GP		bind		selectively			p54	GP			Ets site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_cell_109_2_169_s_255	12007404	A critical test of the ability of METS to discriminate between monomeric sites in cell cycle-regulatory genes and composite elements in cell type-specific genes was provided by ChIP assays, which clearly established selective binding of METS to Ets sites in the  c-Myc,  Cdc2, and  p54 promoters, but not to the composite AP-1/Ets site in the  SR-A promoter in terminally differentiated macrophages.	bind
34162	3	9830	6	11	NULL	NULL	NULL	METS	GP		bind		selectively			Cdc2	GP			Ets site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_cell_109_2_169_s_255	12007404	A critical test of the ability of METS to discriminate between monomeric sites in cell cycle-regulatory genes and composite elements in cell type-specific genes was provided by ChIP assays, which clearly established selective binding of METS to Ets sites in the  c-Myc,  Cdc2, and  p54 promoters, but not to the composite AP-1/Ets site in the  SR-A promoter in terminally differentiated macrophages.	bind
34163	4	9830	6	11	NULL	NULL	NULL	METS	GP		does not bind					SR-A	GP			composite AP-1/Ets site of promoter	NULL	terminally differentiated macrophages	NULL	NULL	NULL	NULL	gw60_cell_109_2_169_s_255	12007404	A critical test of the ability of METS to discriminate between monomeric sites in cell cycle-regulatory genes and composite elements in cell type-specific genes was provided by ChIP assays, which clearly established selective binding of METS to Ets sites in the  c-Myc,  Cdc2, and  p54 promoters, but not to the composite AP-1/Ets site in the  SR-A promoter in terminally differentiated macrophages.	bind
41145	1	9830	7	11	NULL	NULL	NULL	 METS	GP		bind		selectively			c-Myc	GP			Ets sites in the promoter	NULL		NULL	NULL	NULL	NULL	gw60_cell_109_2_169_s_255	12007404	A critical test of the ability of METS to discriminate between monomeric sites in cell cycle-regulatory genes and composite elements in cell type-specific genes was provided by ChIP assays, which clearly established selective binding of METS to Ets sites in the  c-Myc,  Cdc2, and  p54 promoters, but not to the composite AP-1/Ets site in the  SR-A promoter in terminally differentiated macrophages.	bind
41146	2	9830	7	11	NULL	NULL	NULL	METS	GP		bind		selectively			Cdc2	GP			Ets sites in the promoter	NULL		NULL	NULL	NULL	NULL	gw60_cell_109_2_169_s_255	12007404	A critical test of the ability of METS to discriminate between monomeric sites in cell cycle-regulatory genes and composite elements in cell type-specific genes was provided by ChIP assays, which clearly established selective binding of METS to Ets sites in the  c-Myc,  Cdc2, and  p54 promoters, but not to the composite AP-1/Ets site in the  SR-A promoter in terminally differentiated macrophages.	bind
41147	3	9830	7	11	NULL	NULL	NULL	METS	GP		bind		selectively			p54	GP			Ets sites in the promoter	NULL		NULL	NULL	NULL	NULL	gw60_cell_109_2_169_s_255	12007404	A critical test of the ability of METS to discriminate between monomeric sites in cell cycle-regulatory genes and composite elements in cell type-specific genes was provided by ChIP assays, which clearly established selective binding of METS to Ets sites in the  c-Myc,  Cdc2, and  p54 promoters, but not to the composite AP-1/Ets site in the  SR-A promoter in terminally differentiated macrophages.	bind
41148	4	9830	7	11	NULL	NULL	NULL	METS	GP		does not bind					SR-A	GP			composite AP-1/Ets site in the promoter	NULL	terminally differentiated macrophages	NULL	NULL	NULL	NULL	gw60_cell_109_2_169_s_255	12007404	A critical test of the ability of METS to discriminate between monomeric sites in cell cycle-regulatory genes and composite elements in cell type-specific genes was provided by ChIP assays, which clearly established selective binding of METS to Ets sites in the  c-Myc,  Cdc2, and  p54 promoters, but not to the composite AP-1/Ets site in the  SR-A promoter in terminally differentiated macrophages.	bind
34164	1	9831	6	11	NULL	NULL	NULL	apolipoprotein	Chemical		bind			B domain		LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_149_s_271	9012650	A cross-species comparison of the apolipoprotein B domain that binds to the LDL receptor.	bind
41149	1	9831	7	11	NULL	NULL	NULL	 apolipoprotein 	Chemical		binds to			B domain		LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_149_s_271	9012650	A cross-species comparison of the apolipoprotein B domain that binds to the LDL receptor.	bind
34715	1	9832	6	11	NULL	NULL	NULL	CRP-cyclic AMP complex	GP		bind					dorf	NucleicAcid	stronger		CRP recognition site	NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-bacteriol_179_9_9139892_s_12	9139892	A CRP  recognition site is associated with each promoter in the crp-dorf intergenic  region; binding of the CRP-cyclic AMP complex to the stronger dorf CRP  recognition site activates transcription from the dorf promoter and represses  transcription from the crp promoter.	bind
34716	2	9832	6	11	NULL	NULL	NULL	statement 1	Process		activates 					dorf 	NucleicAcid	transcription of		promoter	NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-bacteriol_179_9_9139892_s_12	9139892	A CRP  recognition site is associated with each promoter in the crp-dorf intergenic  region; binding of the CRP-cyclic AMP complex to the stronger dorf CRP  recognition site activates transcription from the dorf promoter and represses  transcription from the crp promoter.	bind
34717	3	9832	6	11	NULL	NULL	NULL	statement 1	Process		represses					crp	GP	transcription of		promoter	NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-bacteriol_179_9_9139892_s_12	9139892	A CRP  recognition site is associated with each promoter in the crp-dorf intergenic  region; binding of the CRP-cyclic AMP complex to the stronger dorf CRP  recognition site activates transcription from the dorf promoter and represses  transcription from the crp promoter.	bind
41150	1	9832	7	11	NULL	NULL	NULL	 CRP-cyclic AMP complex 	GP		bind					dorf	NucleicAcid	stronger		CRP recognition site	NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-bacteriol_179_9_9139892_s_12	9139892	A CRP  recognition site is associated with each promoter in the crp-dorf intergenic  region; binding of the CRP-cyclic AMP complex to the stronger dorf CRP  recognition site activates transcription from the dorf promoter and represses  transcription from the crp promoter.	bind
41151	2	9832	7	11	NULL	NULL	NULL	statement 1	Process		activates					dorf	NucleicAcid	transcription of		promoter	NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-bacteriol_179_9_9139892_s_12	9139892	A CRP  recognition site is associated with each promoter in the crp-dorf intergenic  region; binding of the CRP-cyclic AMP complex to the stronger dorf CRP  recognition site activates transcription from the dorf promoter and represses  transcription from the crp promoter.	bind
41152	3	9832	7	11	NULL	NULL	NULL	statement 1	Process		repress					crp	GP	transcription of		promoter	NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-bacteriol_179_9_9139892_s_12	9139892	A CRP  recognition site is associated with each promoter in the crp-dorf intergenic  region; binding of the CRP-cyclic AMP complex to the stronger dorf CRP  recognition site activates transcription from the dorf promoter and represses  transcription from the crp promoter.	bind
34165	1	9833	6	11	NULL	NULL	NULL	SWI5	GP		encodes					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_84_5_687_s_34	8625407	A crucial role in directing mother cell - specific  HO expression  has been established for the transcription factor encoded by  SWI5 (Nasmyth, 1993   ).	bind
34166	2	9833	6	11	NULL	NULL	NULL	SWI5	GP		directs					HO	GP	expression of;; mother cell-specific			NULL		NULL	NULL	NULL	NULL	gw60_cell_84_5_687_s_34	8625407	A crucial role in directing mother cell - specific  HO expression  has been established for the transcription factor encoded by  SWI5 (Nasmyth, 1993   ).	bind
41153	1	9833	7	11	NULL	NULL	NULL	SWI5 	GP		encodes					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_84_5_687_s_34	8625407	A crucial role in directing mother cell - specific  HO expression  has been established for the transcription factor encoded by  SWI5 (Nasmyth, 1993   ).	bind
56897	2	9833	7	11	NULL	NULL	NULL	SWI5	GP		directs					HO	GP	expression of;; mother cell-specific			NULL		NULL	NULL	NULL	NULL	gw60_cell_84_5_687_s_34	8625407	A crucial role in directing mother cell - specific  HO expression  has been established for the transcription factor encoded by  SWI5 (Nasmyth, 1993   ).	bind
34208	1	9835	6	11	NULL	NULL	NULL	Adk	GP	B.stearothermophilus	bind					Ap5A plus magnesium	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_4_1073_s_184	11842120	A crystal structure of  B.stearothermophilus Adk bound to Ap5A plus magnesium or manganese showed that the Asp and Arg side chains both form hydrogen bonds to a water molecule within the octahedral coordination sphere of the metal ion ( 18).	bind
34211	2	9835	6	11	NULL	NULL	NULL	Adk	GP	B.stearothermophilus	bind					Ap5A plus manganese	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_4_1073_s_184	11842120	A crystal structure of  B.stearothermophilus Adk bound to Ap5A plus magnesium or manganese showed that the Asp and Arg side chains both form hydrogen bonds to a water molecule within the octahedral coordination sphere of the metal ion ( 18).	bind
34213	3	9835	6	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_4_1073_s_184	11842120	A crystal structure of  B.stearothermophilus Adk bound to Ap5A plus magnesium or manganese showed that the Asp and Arg side chains both form hydrogen bonds to a water molecule within the octahedral coordination sphere of the metal ion ( 18).	bind
34217	4	9835	6	11	NULL	NULL	NULL				form hydrogen bonds with			Asp side chains		water molecule	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_4_1073_s_184	11842120	A crystal structure of  B.stearothermophilus Adk bound to Ap5A plus magnesium or manganese showed that the Asp and Arg side chains both form hydrogen bonds to a water molecule within the octahedral coordination sphere of the metal ion ( 18).	bind
34218	5	9835	6	11	NULL	NULL	NULL				form hydrogen bonds with			Arg side chains		water molecule	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_4_1073_s_184	11842120	A crystal structure of  B.stearothermophilus Adk bound to Ap5A plus magnesium or manganese showed that the Asp and Arg side chains both form hydrogen bonds to a water molecule within the octahedral coordination sphere of the metal ion ( 18).	bind
41154	1	9835	7	11	NULL	NULL	NULL	Adk	GP	B.stearothermophilus 	bind					Ap5A plus magnesium	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_4_1073_s_184	11842120	A crystal structure of  B.stearothermophilus Adk bound to Ap5A plus magnesium or manganese showed that the Asp and Arg side chains both form hydrogen bonds to a water molecule within the octahedral coordination sphere of the metal ion ( 18).	bind
41155	2	9835	7	11	NULL	NULL	NULL	Adk	GP	B.stearothermophilus 	bind					Ap5A plus manganese	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_4_1073_s_184	11842120	A crystal structure of  B.stearothermophilus Adk bound to Ap5A plus magnesium or manganese showed that the Asp and Arg side chains both form hydrogen bonds to a water molecule within the octahedral coordination sphere of the metal ion ( 18).	bind
41156	3	9835	7	11	NULL	NULL	NULL	Ap5A	Chemical		forms hydrogen bond with			Asp side chain		water molecule	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_4_1073_s_184	11842120	A crystal structure of  B.stearothermophilus Adk bound to Ap5A plus magnesium or manganese showed that the Asp and Arg side chains both form hydrogen bonds to a water molecule within the octahedral coordination sphere of the metal ion ( 18).	bind
41157	4	9835	7	11	NULL	NULL	NULL	Ap5A	Chemical		forms hydrogen bond with			Arg side chain		water molecule	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_4_1073_s_184	11842120	A crystal structure of  B.stearothermophilus Adk bound to Ap5A plus magnesium or manganese showed that the Asp and Arg side chains both form hydrogen bonds to a water molecule within the octahedral coordination sphere of the metal ion ( 18).	bind
48905	5	9835	7	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_4_1073_s_184	11842120	A crystal structure of  B.stearothermophilus Adk bound to Ap5A plus magnesium or manganese showed that the Asp and Arg side chains both form hydrogen bonds to a water molecule within the octahedral coordination sphere of the metal ion ( 18).	bind
34220	1	9836	6	11	NULL	NULL	NULL	HMGB1	GP		bind			domain A		DNA duplex	NucleicAcid	cisplatin-modified			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_47_43589_s_242	11568187	A crystal structure of HMGB1 domain A bound to a cisplatin-modified DNA duplex revealed the intercalation of a single phenylalanine residue into the hydrophobic wedge created in the minor groove across from the platinum-induced d(GpG) cross-link, with its binding extending mainly to 3' side of the adduct ( 58).	bind
41161	1	9836	7	11	NULL	NULL	NULL	HMGB1	GP		bind			domain A		 DNA duplex	NucleicAcid	cisplatin-modified			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_47_43589_s_242	11568187	A crystal structure of HMGB1 domain A bound to a cisplatin-modified DNA duplex revealed the intercalation of a single phenylalanine residue into the hydrophobic wedge created in the minor groove across from the platinum-induced d(GpG) cross-link, with its binding extending mainly to 3' side of the adduct ( 58).	bind
41165	2	9836	7	11	NULL	NULL	NULL	statement 1	Process		reveals							intercalation of	 phenylalanine residue		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_47_43589_s_242	11568187	A crystal structure of HMGB1 domain A bound to a cisplatin-modified DNA duplex revealed the intercalation of a single phenylalanine residue into the hydrophobic wedge created in the minor groove across from the platinum-induced d(GpG) cross-link, with its binding extending mainly to 3' side of the adduct ( 58).	bind
41173	3	9836	7	11	NULL	NULL	NULL	statement 2	Process		occurs in					minor groove	NucleicAcid	hydrophobic wedge of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_47_43589_s_242	11568187	A crystal structure of HMGB1 domain A bound to a cisplatin-modified DNA duplex revealed the intercalation of a single phenylalanine residue into the hydrophobic wedge created in the minor groove across from the platinum-induced d(GpG) cross-link, with its binding extending mainly to 3' side of the adduct ( 58).	bind
41178	4	9836	7	11	NULL	NULL	NULL	platinum	Chemical		induce					d(GpG) cross-link	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_47_43589_s_242	11568187	A crystal structure of HMGB1 domain A bound to a cisplatin-modified DNA duplex revealed the intercalation of a single phenylalanine residue into the hydrophobic wedge created in the minor groove across from the platinum-induced d(GpG) cross-link, with its binding extending mainly to 3' side of the adduct ( 58).	bind
41179	5	9836	7	11	NULL	NULL	NULL	statement 3	Process		occurs from					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_47_43589_s_242	11568187	A crystal structure of HMGB1 domain A bound to a cisplatin-modified DNA duplex revealed the intercalation of a single phenylalanine residue into the hydrophobic wedge created in the minor groove across from the platinum-induced d(GpG) cross-link, with its binding extending mainly to 3' side of the adduct ( 58).	bind
41180	6	9836	7	11	NULL	NULL	NULL	statement 5	Process		extend to					adduct	Process			3' side of 	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_47_43589_s_242	11568187	A crystal structure of HMGB1 domain A bound to a cisplatin-modified DNA duplex revealed the intercalation of a single phenylalanine residue into the hydrophobic wedge created in the minor groove across from the platinum-induced d(GpG) cross-link, with its binding extending mainly to 3' side of the adduct ( 58).	bind
34224	1	9837	6	11	NULL	NULL	NULL	IleRS	NucleicAcid		bind					tRNAIle	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_23978_s_23	15845536	A crystal structure of IleRS bound to tRNAIle showed that the 3''-end of the tRNA approaches the editing domain, suggesting a plausible structural mechanism in which the flexible 3''-end of misaminoacylated Val-tRNAIle translocates across the enzyme surface from the Rossmann fold domain into the distant editing active site ( ).	bind
34712	2	9837	6	11	NULL	NULL	NULL	Val-tRNAIle 	NucleicAcid	3''-end of;;misaminoacylated	translocates from								Rossmann fold domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_23978_s_23	15845536	A crystal structure of IleRS bound to tRNAIle showed that the 3''-end of the tRNA approaches the editing domain, suggesting a plausible structural mechanism in which the flexible 3''-end of misaminoacylated Val-tRNAIle translocates across the enzyme surface from the Rossmann fold domain into the distant editing active site ( ).	bind
34713	3	9837	6	11	NULL	NULL	NULL	Val-tRNAIle	NucleicAcid	3''-end of;;misaminoacylated	translocates to					distant editing active site	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_23978_s_23	15845536	A crystal structure of IleRS bound to tRNAIle showed that the 3''-end of the tRNA approaches the editing domain, suggesting a plausible structural mechanism in which the flexible 3''-end of misaminoacylated Val-tRNAIle translocates across the enzyme surface from the Rossmann fold domain into the distant editing active site ( ).	bind
34714	4	9837	6	11	NULL	NULL	NULL	statement 3	Process		occurs after					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_23978_s_23	15845536	A crystal structure of IleRS bound to tRNAIle showed that the 3''-end of the tRNA approaches the editing domain, suggesting a plausible structural mechanism in which the flexible 3''-end of misaminoacylated Val-tRNAIle translocates across the enzyme surface from the Rossmann fold domain into the distant editing active site ( ).	bind
41181	1	9837	7	11	NULL	NULL	NULL	IleRS	NucleicAcid		bind					tRNAIle	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_23978_s_23	15845536	A crystal structure of IleRS bound to tRNAIle showed that the 3''-end of the tRNA approaches the editing domain, suggesting a plausible structural mechanism in which the flexible 3''-end of misaminoacylated Val-tRNAIle translocates across the enzyme surface from the Rossmann fold domain into the distant editing active site ( ).	bind
41182	2	9837	7	11	NULL	NULL	NULL	tRNA	NucleicAcid	3'' end of	approaches					editing domain	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_23978_s_23	15845536	A crystal structure of IleRS bound to tRNAIle showed that the 3''-end of the tRNA approaches the editing domain, suggesting a plausible structural mechanism in which the flexible 3''-end of misaminoacylated Val-tRNAIle translocates across the enzyme surface from the Rossmann fold domain into the distant editing active site ( ).	bind
41183	3	9837	7	11	NULL	NULL	NULL	Val-tRNAIle	NucleicAcid	3" end of;;misaminoacylated	translocates across					enzyme surface	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_23978_s_23	15845536	A crystal structure of IleRS bound to tRNAIle showed that the 3''-end of the tRNA approaches the editing domain, suggesting a plausible structural mechanism in which the flexible 3''-end of misaminoacylated Val-tRNAIle translocates across the enzyme surface from the Rossmann fold domain into the distant editing active site ( ).	bind
41184	4	9837	7	11	NULL	NULL	NULL	statement 3	NucleicAcid		translocates from								Rossmann fold domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_23978_s_23	15845536	A crystal structure of IleRS bound to tRNAIle showed that the 3''-end of the tRNA approaches the editing domain, suggesting a plausible structural mechanism in which the flexible 3''-end of misaminoacylated Val-tRNAIle translocates across the enzyme surface from the Rossmann fold domain into the distant editing active site ( ).	bind
41185	5	9837	7	11	NULL	NULL	NULL	statement 4	NucleicAcid		translocates to					distant editing active site	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_23978_s_23	15845536	A crystal structure of IleRS bound to tRNAIle showed that the 3''-end of the tRNA approaches the editing domain, suggesting a plausible structural mechanism in which the flexible 3''-end of misaminoacylated Val-tRNAIle translocates across the enzyme surface from the Rossmann fold domain into the distant editing active site ( ).	bind
34225	1	9838	6	11	NULL	NULL	NULL	SK	GP		plays a role in			beta domain		Pg substrate	GP	processing of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_16_9168_s_72	12878727	A crystal structure of Pg substrate bound to the SK - plasmin complex  has not been obtained, but previous studies have indicated that the SK beta  domain plays a central role in processing Pg substrate  ( ,   ,   ).	bind
41187	1	9838	7	11	NULL	NULL	NULL	SK 	GP		plays a role in			beta domain		Pg substrate	GP	processing of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_16_9168_s_72	12878727	A crystal structure of Pg substrate bound to the SK - plasmin complex  has not been obtained, but previous studies have indicated that the SK beta  domain plays a central role in processing Pg substrate  ( ,   ,   ).	bind
34229	1	9839	6	11	NULL	NULL	NULL				bind			alpha2-I domain		collagen like peptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_13_9985_s_28	11098050	A crystal structure of the alpha2-I domain reveals binding of a collagen-like peptide to a groove in the surface of the "`top"` face of the domain ( 12).	bind
41188	1	9839	7	11	NULL	NULL	NULL				bind			alpha2-I domain 		collagen-like peptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_13_9985_s_28	11098050	A crystal structure of the alpha2-I domain reveals binding of a collagen-like peptide to a groove in the surface of the "`top"` face of the domain ( 12).	bind
34241	1	9840	6	11	NULL	NULL	NULL	gp43	GP		bind			C-terminal 		gp45	GP	bacteriophage RB69	hydrophobic pocket		NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_15_8368_s_242	11459977	A crystal structure of the C-terminal peptide of gp43 bound to gp45 of bacteriophage RB69 shows that the peptide binds away from the subunit interface in a hydrophobic pocket close to the interdomain connecting loop ( 9).	bind
48970	2	9840	6	11	NULL	NULL	NULL				occurs close to			hydrophobic pocket					interdomain connecting loop		NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_15_8368_s_242	11459977	A crystal structure of the C-terminal peptide of gp43 bound to gp45 of bacteriophage RB69 shows that the peptide binds away from the subunit interface in a hydrophobic pocket close to the interdomain connecting loop ( 9).	bind
48971	3	9840	6	11	NULL	NULL	NULL	statement 1	Process		occurs away from								subunit interface		NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_15_8368_s_242	11459977	A crystal structure of the C-terminal peptide of gp43 bound to gp45 of bacteriophage RB69 shows that the peptide binds away from the subunit interface in a hydrophobic pocket close to the interdomain connecting loop ( 9).	bind
41189	1	9840	7	11	NULL	NULL	NULL	gp43	GP		bind			C-terminal peptide of		gp45	GP	bacteriophage RB69	hydrophobic pocket		NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_15_8368_s_242	11459977	A crystal structure of the C-terminal peptide of gp43 bound to gp45 of bacteriophage RB69 shows that the peptide binds away from the subunit interface in a hydrophobic pocket close to the interdomain connecting loop ( 9).	bind
41190	2	9840	7	11	NULL	NULL	NULL	statement 1	Process		occurs away from					 			subunit interface		NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_15_8368_s_242	11459977	A crystal structure of the C-terminal peptide of gp43 bound to gp45 of bacteriophage RB69 shows that the peptide binds away from the subunit interface in a hydrophobic pocket close to the interdomain connecting loop ( 9).	bind
41191	3	9840	7	11	NULL	NULL	NULL				occurs close to			hydrophobic pocket					interdomain connecting loop		NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_15_8368_s_242	11459977	A crystal structure of the C-terminal peptide of gp43 bound to gp45 of bacteriophage RB69 shows that the peptide binds away from the subunit interface in a hydrophobic pocket close to the interdomain connecting loop ( 9).	bind
34242	1	9841	6	11	NULL	NULL	NULL	NF-kappaB p50/p65 heterodimer	GP		bind					Ig-kappaB DNA target	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24392_s_36	10825175	A crystal structure of the NF-kappaB p50/p65 heterodimer bound to the Ig-kappaB DNA target has been completed ( 11).	bind
41198	1	9841	7	11	NULL	NULL	NULL	NF-kappaB p50/p65 heterodimer	GP		bind					Ig-kappaB DNA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24392_s_36	10825175	A crystal structure of the NF-kappaB p50/p65 heterodimer bound to the Ig-kappaB DNA target has been completed ( 11).	bind
34243	1	9842	6	11	NULL	NULL	NULL	A1	GP		bind			RBD		telomeric repeat DNA	NucleicAcid			d(TTAGGG)2	NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_72_0_291_s_334	12626338	A crystal structure of the two RBDs of A1 bound to the telomeric repeat DNA d(TTAGGG)2 shows that an A1 protein dimer forms a four-RNP-domain surface, which binds two DNAs  or four copies of the element ( 156).	bind
34711	2	9842	6	11	NULL	NULL	NULL	A1 protein dimer	GP		forms a 					four-RNP-domain surface	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_72_0_291_s_334	12626338	A crystal structure of the two RBDs of A1 bound to the telomeric repeat DNA d(TTAGGG)2 shows that an A1 protein dimer forms a four-RNP-domain surface, which binds two DNAs  or four copies of the element ( 156).	bind
41199	1	9842	7	11	NULL	NULL	NULL	A1	GP		bind			RBDs		telomeric repeat DNA 	NucleicAcid			d(TTAGGG)2	NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_72_0_291_s_334	12626338	A crystal structure of the two RBDs of A1 bound to the telomeric repeat DNA d(TTAGGG)2 shows that an A1 protein dimer forms a four-RNP-domain surface, which binds two DNAs  or four copies of the element ( 156).	bind
41200	2	9842	7	11	NULL	NULL	NULL	A1 protein dimer	GP		forms					RNP-domain surface	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_72_0_291_s_334	12626338	A crystal structure of the two RBDs of A1 bound to the telomeric repeat DNA d(TTAGGG)2 shows that an A1 protein dimer forms a four-RNP-domain surface, which binds two DNAs  or four copies of the element ( 156).	bind
34244	1	9843	6	11	NULL	NULL	NULL	PP2A	GP		bind					AR	GP		DBD-hinge-LBD region		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_4_1298_s_295	15684382	A crystallographic analysis will be required to determine how the AF-1 phosphorylation sites are spatially positioned relative to the DBD-hinge-LBD region where PP2A binds AR.	bind
41202	1	9843	7	11	NULL	NULL	NULL	PP2A	GP		binds					AR	GP		DBD-hinge-LBD region		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_4_1298_s_295	15684382	A crystallographic analysis will be required to determine how the AF-1 phosphorylation sites are spatially positioned relative to the DBD-hinge-LBD region where PP2A binds AR.	bind
34245	1	9845	6	11	NULL	NULL	NULL	water molecule	Chemical		bind					Csp3	GP		arginine		NULL		NULL	NULL	NULL	NULL	gw60_chembiol_7_6_423_s_109	10873833	A crystallographic water molecule is observed binding to the conserved arginine for Csp3, Csp7 and Csp8.	bind
34252	2	9845	6	11	NULL	NULL	NULL	water molecule	Chemical		bind					Csp7	GP		arginine		NULL		NULL	NULL	NULL	NULL	gw60_chembiol_7_6_423_s_109	10873833	A crystallographic water molecule is observed binding to the conserved arginine for Csp3, Csp7 and Csp8.	bind
34253	3	9845	6	11	NULL	NULL	NULL	water molecule	Chemical		bind					Csp8	GP		arginine		NULL		NULL	NULL	NULL	NULL	gw60_chembiol_7_6_423_s_109	10873833	A crystallographic water molecule is observed binding to the conserved arginine for Csp3, Csp7 and Csp8.	bind
41203	1	9845	7	11	NULL	NULL	NULL	water molecule	Chemical		binds					Csp3	GP		arginine		NULL		NULL	NULL	NULL	NULL	gw60_chembiol_7_6_423_s_109	10873833	A crystallographic water molecule is observed binding to the conserved arginine for Csp3, Csp7 and Csp8.	bind
41204	2	9845	7	11	NULL	NULL	NULL	water molecule	Chemical		binds					Csp7	GP		arginine		NULL		NULL	NULL	NULL	NULL	gw60_chembiol_7_6_423_s_109	10873833	A crystallographic water molecule is observed binding to the conserved arginine for Csp3, Csp7 and Csp8.	bind
41205	3	9845	7	11	NULL	NULL	NULL	water molecule	Chemical		binds					Csp8	GP		arginine		NULL		NULL	NULL	NULL	NULL	gw60_chembiol_7_6_423_s_109	10873833	A crystallographic water molecule is observed binding to the conserved arginine for Csp3, Csp7 and Csp8.	bind
34254	1	9847	6	11	NULL	NULL	NULL	HRGP	GP		bind					TSP-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_107_1_45_s_80	11134179	A CSVTCG-containing peptide from the third type 1 repeat had similar inhibitory activity, but mutated peptides with substitution of alanine for the cysteine residues in the CSVTCG motif did not inhibit HRGP binding to TSP-1.	bind
34255	2	9847	6	11	NULL	NULL	NULL	alanine	AminoAcid		is substituted to					cysteine	AminoAcid		CSVTCG motif		NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_107_1_45_s_80	11134179	A CSVTCG-containing peptide from the third type 1 repeat had similar inhibitory activity, but mutated peptides with substitution of alanine for the cysteine residues in the CSVTCG motif did not inhibit HRGP binding to TSP-1.	bind
34256	3	9847	6	11	NULL	NULL	NULL	statement 2	Process		does not inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_107_1_45_s_80	11134179	A CSVTCG-containing peptide from the third type 1 repeat had similar inhibitory activity, but mutated peptides with substitution of alanine for the cysteine residues in the CSVTCG motif did not inhibit HRGP binding to TSP-1.	bind
34257	4	9847	6	11	NULL	NULL	NULL	CSVTCG-containing peptide	AminoAcid		inhibits			third type 1 repeat		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_107_1_45_s_80	11134179	A CSVTCG-containing peptide from the third type 1 repeat had similar inhibitory activity, but mutated peptides with substitution of alanine for the cysteine residues in the CSVTCG motif did not inhibit HRGP binding to TSP-1.	bind
41210	1	9847	7	11	NULL	NULL	NULL	HRGP	GP		bind					TSP-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_107_1_45_s_80	11134179	A CSVTCG-containing peptide from the third type 1 repeat had similar inhibitory activity, but mutated peptides with substitution of alanine for the cysteine residues in the CSVTCG motif did not inhibit HRGP binding to TSP-1.	bind
41211	2	9847	7	11	NULL	NULL	NULL	CSVTCG-containing peptide	AminoAcid		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_107_1_45_s_80	11134179	A CSVTCG-containing peptide from the third type 1 repeat had similar inhibitory activity, but mutated peptides with substitution of alanine for the cysteine residues in the CSVTCG motif did not inhibit HRGP binding to TSP-1.	bind
41212	4	9847	7	11	NULL	NULL	NULL	statement 3	Process		does not inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_107_1_45_s_80	11134179	A CSVTCG-containing peptide from the third type 1 repeat had similar inhibitory activity, but mutated peptides with substitution of alanine for the cysteine residues in the CSVTCG motif did not inhibit HRGP binding to TSP-1.	bind
41213	5	9847	7	11	NULL	NULL	NULL	third type 1 repeat	AminoAcid		contains					CSVTCG-containing peptide 	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_107_1_45_s_80	11134179	A CSVTCG-containing peptide from the third type 1 repeat had similar inhibitory activity, but mutated peptides with substitution of alanine for the cysteine residues in the CSVTCG motif did not inhibit HRGP binding to TSP-1.	bind
48972	3	9847	7	11	NULL	NULL	NULL	alanine	AminoAcid		is substituted to					cysteine	AminoAcid		CSVTCG motif		NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_107_1_45_s_80	11134179	A CSVTCG-containing peptide from the third type 1 repeat had similar inhibitory activity, but mutated peptides with substitution of alanine for the cysteine residues in the CSVTCG motif did not inhibit HRGP binding to TSP-1.	bind
34258	1	9848	6	11	NULL	NULL	NULL	CtBP dimer	GP		bind					Knirps	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_49_40757_s_142	16186109	A CtBP dimer binding to Knirps would be expected to produce a complex of only  150 kDa; therefore, we tested for the presence of additional proteins using antibodies to candidate proteins.	bind
41214	1	9848	7	11	NULL	NULL	NULL	CtBP dimer	GP		bind					Knirps	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_49_40757_s_142	16186109	A CtBP dimer binding to Knirps would be expected to produce a complex of only  150 kDa; therefore, we tested for the presence of additional proteins using antibodies to candidate proteins.	bind
34259	1	9849	6	11	NULL	NULL	NULL	CTD peptide	AminoAcid	phosphorylated 	bind			S5-repeats		GTase	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1577_2_308_s_93	12213660	A CTD peptide carrying as few as two S5-phosphorylated repeats is sufficient to bind to and stimulate the GTase, whereas peptides phosphorylated at S2 allow GTase binding but no stimulation [ 57].	bind
34260	2	9849	6	11	NULL	NULL	NULL	statement 1	Process		stimulate					GTase	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1577_2_308_s_93	12213660	A CTD peptide carrying as few as two S5-phosphorylated repeats is sufficient to bind to and stimulate the GTase, whereas peptides phosphorylated at S2 allow GTase binding but no stimulation [ 57].	bind
34261	3	9849	6	11	NULL	NULL	NULL	CTD peptide	AminoAcid	phosphorylated	bind			S2 repeats		GTase	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1577_2_308_s_93	12213660	A CTD peptide carrying as few as two S5-phosphorylated repeats is sufficient to bind to and stimulate the GTase, whereas peptides phosphorylated at S2 allow GTase binding but no stimulation [ 57].	bind
34262	4	9849	6	11	NULL	NULL	NULL	statement 3	Process		does not stimulate					GTase	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1577_2_308_s_93	12213660	A CTD peptide carrying as few as two S5-phosphorylated repeats is sufficient to bind to and stimulate the GTase, whereas peptides phosphorylated at S2 allow GTase binding but no stimulation [ 57].	bind
41215	1	9849	7	11	NULL	NULL	NULL	CTD peptide	AminoAcid	phosphorylated	bind			S5-repeats		GTase	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1577_2_308_s_93	12213660	A CTD peptide carrying as few as two S5-phosphorylated repeats is sufficient to bind to and stimulate the GTase, whereas peptides phosphorylated at S2 allow GTase binding but no stimulation [ 57].	bind
41216	2	9849	7	11	NULL	NULL	NULL	statement 1	Process		stimulate					GTase	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1577_2_308_s_93	12213660	A CTD peptide carrying as few as two S5-phosphorylated repeats is sufficient to bind to and stimulate the GTase, whereas peptides phosphorylated at S2 allow GTase binding but no stimulation [ 57].	bind
41217	3	9849	7	11	NULL	NULL	NULL	CTD peptide	AminoAcid	phosphorylated	bind			S2 repeats		GTase	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1577_2_308_s_93	12213660	A CTD peptide carrying as few as two S5-phosphorylated repeats is sufficient to bind to and stimulate the GTase, whereas peptides phosphorylated at S2 allow GTase binding but no stimulation [ 57].	bind
41218	4	9849	7	11	NULL	NULL	NULL	statement 3	Process		does not stimulate					GTase	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1577_2_308_s_93	12213660	A CTD peptide carrying as few as two S5-phosphorylated repeats is sufficient to bind to and stimulate the GTase, whereas peptides phosphorylated at S2 allow GTase binding but no stimulation [ 57].	bind
34263	1	9850	6	11	NULL	NULL	NULL	CTLA-4Ig	GP		bind					B7-1	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-exp-med_184_5_8920853_s_11	8920853	A CTLA-4Ig fusion protein  which binds to both B7-1 and B7-2 was shown to completely block the rescue  of thymocytes from glucocorticoid-induced cell death.	bind
34264	2	9850	6	11	NULL	NULL	NULL	CTLA-4Ig	GP		bind					B7-2	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-exp-med_184_5_8920853_s_11	8920853	A CTLA-4Ig fusion protein  which binds to both B7-1 and B7-2 was shown to completely block the rescue  of thymocytes from glucocorticoid-induced cell death.	bind
34265	3	9850	6	11	NULL	NULL	NULL	thymocytes	Cell		is rescued from					statement 6	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-exp-med_184_5_8920853_s_11	8920853	A CTLA-4Ig fusion protein  which binds to both B7-1 and B7-2 was shown to completely block the rescue  of thymocytes from glucocorticoid-induced cell death.	bind
34266	4	9850	6	11	NULL	NULL	NULL	CTLA-4Ig	GP		blocks		completely			statement 3	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-exp-med_184_5_8920853_s_11	8920853	A CTLA-4Ig fusion protein  which binds to both B7-1 and B7-2 was shown to completely block the rescue  of thymocytes from glucocorticoid-induced cell death.	bind
48973	5	9850	6	11	NULL	NULL	NULL	CTLA-4Ig	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-exp-med_184_5_8920853_s_11	8920853	A CTLA-4Ig fusion protein  which binds to both B7-1 and B7-2 was shown to completely block the rescue  of thymocytes from glucocorticoid-induced cell death.	bind
48975	6	9850	6	11	NULL	NULL	NULL	glucocorticoid	Chemical		induce					cell death	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-exp-med_184_5_8920853_s_11	8920853	A CTLA-4Ig fusion protein  which binds to both B7-1 and B7-2 was shown to completely block the rescue  of thymocytes from glucocorticoid-induced cell death.	bind
41219	1	9850	7	11	NULL	NULL	NULL	CTLA-4Ig	GP		binds to					 B7-1	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-exp-med_184_5_8920853_s_11	8920853	A CTLA-4Ig fusion protein  which binds to both B7-1 and B7-2 was shown to completely block the rescue  of thymocytes from glucocorticoid-induced cell death.	bind
41220	2	9850	7	11	NULL	NULL	NULL	CTLA-4Ig	GP		binds to					B7-2	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-exp-med_184_5_8920853_s_11	8920853	A CTLA-4Ig fusion protein  which binds to both B7-1 and B7-2 was shown to completely block the rescue  of thymocytes from glucocorticoid-induced cell death.	bind
41221	3	9850	7	11	NULL	NULL	NULL	glucocorticoid	Chemical		induce					cell death	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-exp-med_184_5_8920853_s_11	8920853	A CTLA-4Ig fusion protein  which binds to both B7-1 and B7-2 was shown to completely block the rescue  of thymocytes from glucocorticoid-induced cell death.	bind
41222	4	9850	7	11	NULL	NULL	NULL	thymocytes	Cell		is rescued from					statement 3	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-exp-med_184_5_8920853_s_11	8920853	A CTLA-4Ig fusion protein  which binds to both B7-1 and B7-2 was shown to completely block the rescue  of thymocytes from glucocorticoid-induced cell death.	bind
41223	5	9850	7	11	NULL	NULL	NULL	CTLA-4Ig	GP		block		completely			statement 4	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-exp-med_184_5_8920853_s_11	8920853	A CTLA-4Ig fusion protein  which binds to both B7-1 and B7-2 was shown to completely block the rescue  of thymocytes from glucocorticoid-induced cell death.	bind
48974	6	9850	7	11	NULL	NULL	NULL	CTLA-4Ig 	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-exp-med_184_5_8920853_s_11	8920853	A CTLA-4Ig fusion protein  which binds to both B7-1 and B7-2 was shown to completely block the rescue  of thymocytes from glucocorticoid-induced cell death.	bind
34706	1	9851	6	11	NULL	NULL	NULL	Chl a	Chemical		is in close contact with					Chl b	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_471_1_89_s_8	10760519	A current 3.4  Ang  structural model of Lhcb1 monomer of the LHCII trimer [  9] includes three membrane spanning helices binding 12 chlorophyll (Chl) molecules with Chl  a in close contact with Chl  b for rapid energy transfer and two crossed lutein molecules possibly quenching Chl  a triplet states.	bind
34707	2	9851	6	11	NULL	NULL	NULL	Lhcb1 monomer	GP		bind			membrane spanning helices		Chl molecules	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_471_1_89_s_8	10760519	A current 3.4  Ang  structural model of Lhcb1 monomer of the LHCII trimer [  9] includes three membrane spanning helices binding 12 chlorophyll (Chl) molecules with Chl  a in close contact with Chl  b for rapid energy transfer and two crossed lutein molecules possibly quenching Chl  a triplet states.	bind
34708	3	9851	6	11	NULL	NULL	NULL	Chl	Chemical		is					chlorophyll	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_471_1_89_s_8	10760519	A current 3.4  Ang  structural model of Lhcb1 monomer of the LHCII trimer [  9] includes three membrane spanning helices binding 12 chlorophyll (Chl) molecules with Chl  a in close contact with Chl  b for rapid energy transfer and two crossed lutein molecules possibly quenching Chl  a triplet states.	bind
34709	4	9851	6	11	NULL	NULL	NULL	statement 1	Process		is needed for					energy transfer	Process	rapid			NULL		NULL	NULL	NULL	NULL	gw60_febslett_471_1_89_s_8	10760519	A current 3.4  Ang  structural model of Lhcb1 monomer of the LHCII trimer [  9] includes three membrane spanning helices binding 12 chlorophyll (Chl) molecules with Chl  a in close contact with Chl  b for rapid energy transfer and two crossed lutein molecules possibly quenching Chl  a triplet states.	bind
34710	5	9851	6	11	NULL	NULL	NULL	leutin molecules	Chemical		quench					Chl a	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_471_1_89_s_8	10760519	A current 3.4  Ang  structural model of Lhcb1 monomer of the LHCII trimer [  9] includes three membrane spanning helices binding 12 chlorophyll (Chl) molecules with Chl  a in close contact with Chl  b for rapid energy transfer and two crossed lutein molecules possibly quenching Chl  a triplet states.	bind
41225	2	9851	7	11	NULL	NULL	NULL	Lhcb1 monomer	GP		bind			membrane spanning helices		Chl molecules	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_471_1_89_s_8	10760519	A current 3.4  Ang  structural model of Lhcb1 monomer of the LHCII trimer [  9] includes three membrane spanning helices binding 12 chlorophyll (Chl) molecules with Chl  a in close contact with Chl  b for rapid energy transfer and two crossed lutein molecules possibly quenching Chl  a triplet states.	bind
41226	3	9851	7	11	NULL	NULL	NULL	Chl a	Chemical		is in close contact with					Chl b	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_471_1_89_s_8	10760519	A current 3.4  Ang  structural model of Lhcb1 monomer of the LHCII trimer [  9] includes three membrane spanning helices binding 12 chlorophyll (Chl) molecules with Chl  a in close contact with Chl  b for rapid energy transfer and two crossed lutein molecules possibly quenching Chl  a triplet states.	bind
41227	4	9851	7	11	NULL	NULL	NULL	statement 3	Process		is needed for					energy transfer	Process	rapid			NULL		NULL	NULL	NULL	NULL	gw60_febslett_471_1_89_s_8	10760519	A current 3.4  Ang  structural model of Lhcb1 monomer of the LHCII trimer [  9] includes three membrane spanning helices binding 12 chlorophyll (Chl) molecules with Chl  a in close contact with Chl  b for rapid energy transfer and two crossed lutein molecules possibly quenching Chl  a triplet states.	bind
41228	5	9851	7	11	NULL	NULL	NULL	lutein molecules	Chemical		quench					Chl a 	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_471_1_89_s_8	10760519	A current 3.4  Ang  structural model of Lhcb1 monomer of the LHCII trimer [  9] includes three membrane spanning helices binding 12 chlorophyll (Chl) molecules with Chl  a in close contact with Chl  b for rapid energy transfer and two crossed lutein molecules possibly quenching Chl  a triplet states.	bind
41230	1	9851	7	11	NULL	NULL	NULL	Chl molecules	Chemical		is					chlorophyll	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_471_1_89_s_8	10760519	A current 3.4  Ang  structural model of Lhcb1 monomer of the LHCII trimer [  9] includes three membrane spanning helices binding 12 chlorophyll (Chl) molecules with Chl  a in close contact with Chl  b for rapid energy transfer and two crossed lutein molecules possibly quenching Chl  a triplet states.	bind
34267	1	9852	6	11	NULL	NULL	NULL	CREB	GP		is					cyclic-AMP response element binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_76_1_7_s_193	10719210	A current cellular theory of depression outlined by Duman et al. [ 21] implicates the cyclic-AMP response element binding protein (CREB) transcription factor as an intracellular target of long but not short term antidepressant treatment.	bind
34268	2	9852	6	11	NULL	NULL	NULL	CREB	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_76_1_7_s_193	10719210	A current cellular theory of depression outlined by Duman et al. [ 21] implicates the cyclic-AMP response element binding protein (CREB) transcription factor as an intracellular target of long but not short term antidepressant treatment.	bind
34269	3	9852	6	11	NULL	NULL	NULL	CREB 	GP		is a target for		intracellular			antidepressant treatment	MedicalFinding	long term			NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_76_1_7_s_193	10719210	A current cellular theory of depression outlined by Duman et al. [ 21] implicates the cyclic-AMP response element binding protein (CREB) transcription factor as an intracellular target of long but not short term antidepressant treatment.	bind
48976	4	9852	6	11	NULL	NULL	NULL	CREB	GP		is not a target for					antidepressant treatment	MedicalFinding	short term			NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_76_1_7_s_193	10719210	A current cellular theory of depression outlined by Duman et al. [ 21] implicates the cyclic-AMP response element binding protein (CREB) transcription factor as an intracellular target of long but not short term antidepressant treatment.	bind
41232	1	9852	7	11	NULL	NULL	NULL	CREB	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_76_1_7_s_193	10719210	A current cellular theory of depression outlined by Duman et al. [ 21] implicates the cyclic-AMP response element binding protein (CREB) transcription factor as an intracellular target of long but not short term antidepressant treatment.	bind
41233	2	9852	7	11	NULL	NULL	NULL	CREB	GP		is					cyclic-AMP response element binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_76_1_7_s_193	10719210	A current cellular theory of depression outlined by Duman et al. [ 21] implicates the cyclic-AMP response element binding protein (CREB) transcription factor as an intracellular target of long but not short term antidepressant treatment.	bind
41235	3	9852	7	11	NULL	NULL	NULL	CREB	GP		is a target for		intracellular			antidepressant treatment	MedicalFinding	long term			NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_76_1_7_s_193	10719210	A current cellular theory of depression outlined by Duman et al. [ 21] implicates the cyclic-AMP response element binding protein (CREB) transcription factor as an intracellular target of long but not short term antidepressant treatment.	bind
41236	4	9852	7	11	NULL	NULL	NULL	CREB	GP		is not a target for					antidepressant treatment	MedicalFinding	short term			NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_76_1_7_s_193	10719210	A current cellular theory of depression outlined by Duman et al. [ 21] implicates the cyclic-AMP response element binding protein (CREB) transcription factor as an intracellular target of long but not short term antidepressant treatment.	bind
34270	1	9853	6	11	NULL	NULL	NULL	Sir1p	GP		bind					HMR-E	GP				NULL	chromatin	NULL	NULL	NULL	NULL	gw60_genesdev_15_2_147_s_45	11157772	A current model for silencing  HMR posits that Sir1p binds to the  HMR-E silencer in chromatin through interactions with the ORC that is bound directly to the silencer ACS.	bind
34271	2	9853	6	11	NULL	NULL	NULL	ORC	GP		bind		directly			ACS	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_2_147_s_45	11157772	A current model for silencing  HMR posits that Sir1p binds to the  HMR-E silencer in chromatin through interactions with the ORC that is bound directly to the silencer ACS.	bind
34272	3	9853	6	11	NULL	NULL	NULL	Sir1p	GP		interacts with					ORC	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_2_147_s_45	11157772	A current model for silencing  HMR posits that Sir1p binds to the  HMR-E silencer in chromatin through interactions with the ORC that is bound directly to the silencer ACS.	bind
48977	4	9853	6	11	NULL	NULL	NULL	statement 1	Process		occurs through					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_2_147_s_45	11157772	A current model for silencing  HMR posits that Sir1p binds to the  HMR-E silencer in chromatin through interactions with the ORC that is bound directly to the silencer ACS.	bind
48978	5	9853	6	11	NULL	NULL	NULL	HMR-E	GP		is a type of					silencer	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_2_147_s_45	11157772	A current model for silencing  HMR posits that Sir1p binds to the  HMR-E silencer in chromatin through interactions with the ORC that is bound directly to the silencer ACS.	bind
48979	6	9853	6	11	NULL	NULL	NULL	ACS	GP		is a type of					silencer	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_2_147_s_45	11157772	A current model for silencing  HMR posits that Sir1p binds to the  HMR-E silencer in chromatin through interactions with the ORC that is bound directly to the silencer ACS.	bind
41239	1	9853	7	11	NULL	NULL	NULL	 Sir1p	GP		binds to					HMR-E	GP				NULL	chromatin	NULL	NULL	NULL	NULL	gw60_genesdev_15_2_147_s_45	11157772	A current model for silencing  HMR posits that Sir1p binds to the  HMR-E silencer in chromatin through interactions with the ORC that is bound directly to the silencer ACS.	bind
41240	2	9853	7	11	NULL	NULL	NULL	ORC 	GP		bind		directly			ACS	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_2_147_s_45	11157772	A current model for silencing  HMR posits that Sir1p binds to the  HMR-E silencer in chromatin through interactions with the ORC that is bound directly to the silencer ACS.	bind
41241	3	9853	7	11	NULL	NULL	NULL	Sir1p	GP		interacts with					ORC	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_2_147_s_45	11157772	A current model for silencing  HMR posits that Sir1p binds to the  HMR-E silencer in chromatin through interactions with the ORC that is bound directly to the silencer ACS.	bind
48980	4	9853	7	11	NULL	NULL	NULL	statement 1	Process		occurs through					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_2_147_s_45	11157772	A current model for silencing  HMR posits that Sir1p binds to the  HMR-E silencer in chromatin through interactions with the ORC that is bound directly to the silencer ACS.	bind
48981	5	9853	7	11	NULL	NULL	NULL	HMR-E	GP		is a type of					silencer	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_2_147_s_45	11157772	A current model for silencing  HMR posits that Sir1p binds to the  HMR-E silencer in chromatin through interactions with the ORC that is bound directly to the silencer ACS.	bind
48982	6	9853	7	11	NULL	NULL	NULL	ACS	GP		is a type of					silencer	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_2_147_s_45	11157772	A current model for silencing  HMR posits that Sir1p binds to the  HMR-E silencer in chromatin through interactions with the ORC that is bound directly to the silencer ACS.	bind
34273	1	9854	6	11	NULL	NULL	NULL	Cdc13p	GP	telomere-associated	bind					Est1p	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_curr-opin-cell-biol_15_3_12787768_s_5	12787768	A current model for telomerase regulation is that  telomere-associated Cdc13p binds Est1p, thereby recruiting telomerase.	bind
34312	2	9854	6	11	NULL	NULL	NULL	statement 1	Process		recruits					telomerase	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_curr-opin-cell-biol_15_3_12787768_s_5	12787768	A current model for telomerase regulation is that  telomere-associated Cdc13p binds Est1p, thereby recruiting telomerase.	bind
41243	1	9854	7	11	NULL	NULL	NULL	Cdc13p	GP	telomere-associated	binds					Est1p	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_curr-opin-cell-biol_15_3_12787768_s_5	12787768	A current model for telomerase regulation is that  telomere-associated Cdc13p binds Est1p, thereby recruiting telomerase.	bind
41244	2	9854	7	11	NULL	NULL	NULL	statement 1	Process		recruits					telomerase	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_curr-opin-cell-biol_15_3_12787768_s_5	12787768	A current model for telomerase regulation is that  telomere-associated Cdc13p binds Est1p, thereby recruiting telomerase.	bind
34314	1	9855	6	11	NULL	NULL	NULL	FNBP	GP		bind					FN	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_74_10_5586_s_289	16988233	A current model for the function of these FNBPs suggested that the binding of FNBP with multiple FNs resulted in the localization of integrin binding sites, which induce the clustering of integrins in the membrane of host cells ( ).	bind
34315	2	9855	6	11	NULL	NULL	NULL	statement 1	Process		resulted in							localization of	integrin binding sites		NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_74_10_5586_s_289	16988233	A current model for the function of these FNBPs suggested that the binding of FNBP with multiple FNs resulted in the localization of integrin binding sites, which induce the clustering of integrins in the membrane of host cells ( ).	bind
34322	3	9855	6	11	NULL	NULL	NULL	statement 2	Process		induce					integrins	GP	clustering of			NULL	membrane of host cells	NULL	NULL	NULL	NULL	gw70_infectimmun_74_10_5586_s_289	16988233	A current model for the function of these FNBPs suggested that the binding of FNBP with multiple FNs resulted in the localization of integrin binding sites, which induce the clustering of integrins in the membrane of host cells ( ).	bind
41246	1	9855	7	11	NULL	NULL	NULL	FNBP	GP		bind					FNs	GP				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_74_10_5586_s_289	16988233	A current model for the function of these FNBPs suggested that the binding of FNBP with multiple FNs resulted in the localization of integrin binding sites, which induce the clustering of integrins in the membrane of host cells ( ).	bind
41248	2	9855	7	11	NULL	NULL	NULL	statement 1	Process		results in							 localization of	integrin binding sites		NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_74_10_5586_s_289	16988233	A current model for the function of these FNBPs suggested that the binding of FNBP with multiple FNs resulted in the localization of integrin binding sites, which induce the clustering of integrins in the membrane of host cells ( ).	bind
41250	3	9855	7	11	NULL	NULL	NULL	statement 2	Process		induce					integrins	GP	clustering of 			NULL	membrane of host cells	NULL	NULL	NULL	NULL	gw70_infectimmun_74_10_5586_s_289	16988233	A current model for the function of these FNBPs suggested that the binding of FNBP with multiple FNs resulted in the localization of integrin binding sites, which induce the clustering of integrins in the membrane of host cells ( ).	bind
34330	1	9856	6	11	NULL	NULL	NULL	GRK	GP		bind					agonist-occupied receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_13266_s_155	8662816	A current model of homologous desensitization of G protein-coupled receptors proposes rapid, agonist-dependent translocation to the plasma membrane of a GRK, which binds and phosphorylates the agonist-occupied receptor ( 2).	bind
34705	2	9856	6	11	NULL	NULL	NULL	statement 1	Process		phosphorylates					agonist-occupied receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_13266_s_155	8662816	A current model of homologous desensitization of G protein-coupled receptors proposes rapid, agonist-dependent translocation to the plasma membrane of a GRK, which binds and phosphorylates the agonist-occupied receptor ( 2).	bind
48983	3	9856	6	11	NULL	NULL	NULL	GRK	GP		translocates to					plasma membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_13266_s_155	8662816	A current model of homologous desensitization of G protein-coupled receptors proposes rapid, agonist-dependent translocation to the plasma membrane of a GRK, which binds and phosphorylates the agonist-occupied receptor ( 2).	bind
48984	4	9856	6	11	NULL	NULL	NULL	statement 3	Process		is dependent on					agonist	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_13266_s_155	8662816	A current model of homologous desensitization of G protein-coupled receptors proposes rapid, agonist-dependent translocation to the plasma membrane of a GRK, which binds and phosphorylates the agonist-occupied receptor ( 2).	bind
41556	1	9856	7	11	NULL	NULL	NULL	GRK	GP		translocates to					plasma membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_13266_s_155	8662816	A current model of homologous desensitization of G protein-coupled receptors proposes rapid, agonist-dependent translocation to the plasma membrane of a GRK, which binds and phosphorylates the agonist-occupied receptor ( 2).	bind
41557	2	9856	7	11	NULL	NULL	NULL	statement 1	Process		is dependent on					agonist	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_13266_s_155	8662816	A current model of homologous desensitization of G protein-coupled receptors proposes rapid, agonist-dependent translocation to the plasma membrane of a GRK, which binds and phosphorylates the agonist-occupied receptor ( 2).	bind
41558	3	9856	7	11	NULL	NULL	NULL	GRK	GP		binds					agonist-occupied receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_13266_s_155	8662816	A current model of homologous desensitization of G protein-coupled receptors proposes rapid, agonist-dependent translocation to the plasma membrane of a GRK, which binds and phosphorylates the agonist-occupied receptor ( 2).	bind
41559	4	9856	7	11	NULL	NULL	NULL	statement 3	Process		phosphorylates					agonist-occupied receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_13266_s_155	8662816	A current model of homologous desensitization of G protein-coupled receptors proposes rapid, agonist-dependent translocation to the plasma membrane of a GRK, which binds and phosphorylates the agonist-occupied receptor ( 2).	bind
34334	1	9860	6	11	NULL	NULL	NULL	ATP	Chemical		bind		preferentially			M2S structural state	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_6_2944_s_163	9501195	A cycle is easily established if ATP binds preferentially to the M2S structural state, which would occur if the transition from M1S to M2S is coupled to a product-release step or is faster than the rate of ADP release.	bind
41563	1	9860	7	11	NULL	NULL	NULL	ATP	Chemical		binds		preferentially			M2S structural state	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_6_2944_s_163	9501195	A cycle is easily established if ATP binds preferentially to the M2S structural state, which would occur if the transition from M1S to M2S is coupled to a product-release step or is faster than the rate of ADP release.	bind
34343	1	9861	6	11	NULL	NULL	NULL	myosin crossbridges	GP		bind					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_102_5_683_s_10	11007486	A cycle of actin - myosin interactions is thought to occur  as follows (Lymn and Taylor, 1971   ;  Spudich, 1994   ): the myosin  crossbridge binds to ATP, and then releases its attached actin filament.	bind
34346	2	9861	6	11	NULL	NULL	NULL	statement 1	Process		releases					actin filament	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_102_5_683_s_10	11007486	A cycle of actin - myosin interactions is thought to occur  as follows (Lymn and Taylor, 1971   ;  Spudich, 1994   ): the myosin  crossbridge binds to ATP, and then releases its attached actin filament.	bind
41568	1	9861	7	11	NULL	NULL	NULL	myosin crossbridge	GP		binds to					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_102_5_683_s_10	11007486	A cycle of actin - myosin interactions is thought to occur  as follows (Lymn and Taylor, 1971   ;  Spudich, 1994   ): the myosin  crossbridge binds to ATP, and then releases its attached actin filament.	bind
41569	2	9861	7	11	NULL	NULL	NULL	statement 1	Process		release					actin filament	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_102_5_683_s_10	11007486	A cycle of actin - myosin interactions is thought to occur  as follows (Lymn and Taylor, 1971   ;  Spudich, 1994   ): the myosin  crossbridge binds to ATP, and then releases its attached actin filament.	bind
34352	3	9862	6	11	NULL	NULL	NULL	statement 1	GP		bind					CREB1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5329_s_5	15964791	A cyclic AMP response element (CRE)-like element in the 5''-flanking region of the MuSK gene binds to CREB1	bind
34353	2	9862	6	11	NULL	NULL	NULL	CRE	GP		is					cyclic-AMP response element	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5329_s_5	15964791	A cyclic AMP response element (CRE)-like element in the 5''-flanking region of the MuSK gene binds to CREB1	bind
56901	1	9862	6	11	NULL	NULL	NULL	MuSK gene	GP		is present in				CRE-like element	MuSK gene	GP	5''-flanking region of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5329_s_5	15964791	A cyclic AMP response element (CRE)-like element in the 5''-flanking region of the MuSK gene binds to CREB1	bind
41572	3	9862	7	11	NULL	NULL	NULL	statement 1	GP		binds to					CREB1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5329_s_5	15964791	A cyclic AMP response element (CRE)-like element in the 5''-flanking region of the MuSK gene binds to CREB1	bind
41573	2	9862	7	11	NULL	NULL	NULL	CRE	GP		is					cyclic AMP response element 	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5329_s_5	15964791	A cyclic AMP response element (CRE)-like element in the 5''-flanking region of the MuSK gene binds to CREB1	bind
56902	1	9862	7	11	NULL	NULL	NULL	MuSK gene	GP		is present in				CRE-like element	MuSK gene	GP	5''-flanking region of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_13_5329_s_5	15964791	A cyclic AMP response element (CRE)-like element in the 5''-flanking region of the MuSK gene binds to CREB1	bind
34356	1	9863	6	11	NULL	NULL	NULL	anti-alpha5 mAb	GP		bind					alpha5beta1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_40_25664_s_5	9748233	A cyclic peptide containing this sequence (*CRRETAWAC*) had little effect on the binding of most anti-alpha5 and anti-beta1 mAbs to alpha5beta1 but completely blocked binding of the anti-alpha5 mAb 16 in a directly competitive manner.	bind
34357	2	9863	6	11	NULL	NULL	NULL	anti-beta1 mAb	GP		bind					alpha5beta1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_40_25664_s_5	9748233	A cyclic peptide containing this sequence (*CRRETAWAC*) had little effect on the binding of most anti-alpha5 and anti-beta1 mAbs to alpha5beta1 but completely blocked binding of the anti-alpha5 mAb 16 in a directly competitive manner.	bind
34703	3	9863	6	11	NULL	NULL	NULL	cyclic peptide	GP		has little effect on			CRRETAWAC		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_40_25664_s_5	9748233	A cyclic peptide containing this sequence (*CRRETAWAC*) had little effect on the binding of most anti-alpha5 and anti-beta1 mAbs to alpha5beta1 but completely blocked binding of the anti-alpha5 mAb 16 in a directly competitive manner.	bind
34704	4	9863	6	11	NULL	NULL	NULL	cyclic peptide	GP		has little effect on			CRRETAWAC		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_40_25664_s_5	9748233	A cyclic peptide containing this sequence (*CRRETAWAC*) had little effect on the binding of most anti-alpha5 and anti-beta1 mAbs to alpha5beta1 but completely blocked binding of the anti-alpha5 mAb 16 in a directly competitive manner.	bind
48985	5	9863	6	11	NULL	NULL	NULL	anti-alpha5 mAb 16	GP		bind					alpha5beta1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_40_25664_s_5	9748233	A cyclic peptide containing this sequence (*CRRETAWAC*) had little effect on the binding of most anti-alpha5 and anti-beta1 mAbs to alpha5beta1 but completely blocked binding of the anti-alpha5 mAb 16 in a directly competitive manner.	bind
48986	6	9863	6	11	NULL	NULL	NULL	cyclic peptide	GP		block		directly;;competitively	CRRETAWAC		statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_40_25664_s_5	9748233	A cyclic peptide containing this sequence (*CRRETAWAC*) had little effect on the binding of most anti-alpha5 and anti-beta1 mAbs to alpha5beta1 but completely blocked binding of the anti-alpha5 mAb 16 in a directly competitive manner.	bind
41576	1	9863	7	11	NULL	NULL	NULL	anti-alpha5 mAb	GP		bind					alpha5beta1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_40_25664_s_5	9748233	A cyclic peptide containing this sequence (*CRRETAWAC*) had little effect on the binding of most anti-alpha5 and anti-beta1 mAbs to alpha5beta1 but completely blocked binding of the anti-alpha5 mAb 16 in a directly competitive manner.	bind
41577	2	9863	7	11	NULL	NULL	NULL	anti-beta1 mAb	GP		bind					alpha5beta1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_40_25664_s_5	9748233	A cyclic peptide containing this sequence (*CRRETAWAC*) had little effect on the binding of most anti-alpha5 and anti-beta1 mAbs to alpha5beta1 but completely blocked binding of the anti-alpha5 mAb 16 in a directly competitive manner.	bind
41578	3	9863	7	11	NULL	NULL	NULL	cyclic peptide 	GP		little effect on			CRRETAWAC		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_40_25664_s_5	9748233	A cyclic peptide containing this sequence (*CRRETAWAC*) had little effect on the binding of most anti-alpha5 and anti-beta1 mAbs to alpha5beta1 but completely blocked binding of the anti-alpha5 mAb 16 in a directly competitive manner.	bind
41579	4	9863	7	11	NULL	NULL	NULL	cyclic peptide 	GP		little effect on			CRRETAWAC		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_40_25664_s_5	9748233	A cyclic peptide containing this sequence (*CRRETAWAC*) had little effect on the binding of most anti-alpha5 and anti-beta1 mAbs to alpha5beta1 but completely blocked binding of the anti-alpha5 mAb 16 in a directly competitive manner.	bind
41580	5	9863	7	11	NULL	NULL	NULL	anti-alpha5 mAb 16	GP		bind					alpha5beta1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_40_25664_s_5	9748233	A cyclic peptide containing this sequence (*CRRETAWAC*) had little effect on the binding of most anti-alpha5 and anti-beta1 mAbs to alpha5beta1 but completely blocked binding of the anti-alpha5 mAb 16 in a directly competitive manner.	bind
41585	6	9863	7	11	NULL	NULL	NULL	cyclic peptide	GP		block		directly;;competitively	CRRETAWAC		statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_40_25664_s_5	9748233	A cyclic peptide containing this sequence (*CRRETAWAC*) had little effect on the binding of most anti-alpha5 and anti-beta1 mAbs to alpha5beta1 but completely blocked binding of the anti-alpha5 mAb 16 in a directly competitive manner.	bind
34359	1	9865	6	11	NULL	NULL	NULL	thrombospondin 1	GP		bind					CD36 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_34_35159_s_145	15192113	A Cys-Ser-Val-Thr-Cys-Gly motif that is suggested to mediate thrombospondin 1 binding to the CD36 receptor ( ) is present at an identical location within TSR4 of human and mouse ADAMTS7B.	bind
34360	2	9865	6	11	NULL	NULL	NULL				mediate			Cys-Ser-Val-Thr-Cys-Gly motif		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_34_35159_s_145	15192113	A Cys-Ser-Val-Thr-Cys-Gly motif that is suggested to mediate thrombospondin 1 binding to the CD36 receptor ( ) is present at an identical location within TSR4 of human and mouse ADAMTS7B.	bind
41603	1	9865	7	11	NULL	NULL	NULL	 thrombospondin 1 	GP		bind					CD36 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_34_35159_s_145	15192113	A Cys-Ser-Val-Thr-Cys-Gly motif that is suggested to mediate thrombospondin 1 binding to the CD36 receptor ( ) is present at an identical location within TSR4 of human and mouse ADAMTS7B.	bind
41604	2	9865	7	11	NULL	NULL	NULL				mediate			Cys-Ser-Val-Thr-Cys-Gly motif		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_34_35159_s_145	15192113	A Cys-Ser-Val-Thr-Cys-Gly motif that is suggested to mediate thrombospondin 1 binding to the CD36 receptor ( ) is present at an identical location within TSR4 of human and mouse ADAMTS7B.	bind
41606	3	9865	7	11	NULL	NULL	NULL				is present			Cys-Ser-Val-Thr-Cys-Gly motif		ADAMTS7B	GP	human	within TSR4 		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_34_35159_s_145	15192113	A Cys-Ser-Val-Thr-Cys-Gly motif that is suggested to mediate thrombospondin 1 binding to the CD36 receptor ( ) is present at an identical location within TSR4 of human and mouse ADAMTS7B.	bind
41607	4	9865	7	11	NULL	NULL	NULL				is present 			Cys-Ser-Val-Thr-Cys-Gly motif		ADAMTS7B	GP	mouse	within TSR4 		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_34_35159_s_145	15192113	A Cys-Ser-Val-Thr-Cys-Gly motif that is suggested to mediate thrombospondin 1 binding to the CD36 receptor ( ) is present at an identical location within TSR4 of human and mouse ADAMTS7B.	bind
34361	1	9866	6	11	NULL	NULL	NULL	CD4 tail	GP		bind			cysteine motif		p56 lck	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_289_5483_1349_s_16	10958781	A cysteine motif present in the CD4 tail binds src-family kinase p56 lck ( 8), and Lck appears to be responsible for phosphorylating CD3zeta, the earliest known event in T cell signaling ( 9).	bind
34362	2	9866	6	11	NULL	NULL	NULL	p56 lck	GP		is a type of					src-family kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_289_5483_1349_s_16	10958781	A cysteine motif present in the CD4 tail binds src-family kinase p56 lck ( 8), and Lck appears to be responsible for phosphorylating CD3zeta, the earliest known event in T cell signaling ( 9).	bind
34363	3	9866	6	11	NULL	NULL	NULL	lck	GP		phosphorylates					CD3zeta	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_289_5483_1349_s_16	10958781	A cysteine motif present in the CD4 tail binds src-family kinase p56 lck ( 8), and Lck appears to be responsible for phosphorylating CD3zeta, the earliest known event in T cell signaling ( 9).	bind
34374	4	9866	6	11	NULL	NULL	NULL	statement 3	Process		is involved in					T cell signaling	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_289_5483_1349_s_16	10958781	A cysteine motif present in the CD4 tail binds src-family kinase p56 lck ( 8), and Lck appears to be responsible for phosphorylating CD3zeta, the earliest known event in T cell signaling ( 9).	bind
41608	1	9866	7	11	NULL	NULL	NULL	CD4 tail	GP		binds			cysteine motif 		p56 lck	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_289_5483_1349_s_16	10958781	A cysteine motif present in the CD4 tail binds src-family kinase p56 lck ( 8), and Lck appears to be responsible for phosphorylating CD3zeta, the earliest known event in T cell signaling ( 9).	bind
41609	2	9866	7	11	NULL	NULL	NULL	p56 lck	GP		is a type of					src-family kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_289_5483_1349_s_16	10958781	A cysteine motif present in the CD4 tail binds src-family kinase p56 lck ( 8), and Lck appears to be responsible for phosphorylating CD3zeta, the earliest known event in T cell signaling ( 9).	bind
41610	3	9866	7	11	NULL	NULL	NULL	Lck	GP		phosphorylate					CD3zeta	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_289_5483_1349_s_16	10958781	A cysteine motif present in the CD4 tail binds src-family kinase p56 lck ( 8), and Lck appears to be responsible for phosphorylating CD3zeta, the earliest known event in T cell signaling ( 9).	bind
41613	4	9866	7	11	NULL	NULL	NULL	statement 3	Process		is involved in					T cell signaling	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_289_5483_1349_s_16	10958781	A cysteine motif present in the CD4 tail binds src-family kinase p56 lck ( 8), and Lck appears to be responsible for phosphorylating CD3zeta, the earliest known event in T cell signaling ( 9).	bind
34701	1	9867	6	11	NULL	NULL	NULL	hCG analog	GP		bind			S138C in the beta-subunit COOH terminus		LHR	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_43_44442_s_376	15304493	A cysteine residue that had been added to the beta-subunit COOH terminus of a bifunctional hCG analog ( i.e. CFC101 - 114,) S138Cthat binds LHR and FSHR was found to become cross-linked to cysteines  added to the alpha-subunit during heterodimer synthesis in COS-7 cells.	bind
34702	2	9867	6	11	NULL	NULL	NULL				bind			S138C in the beta-subunit COOH terminus		FSHR	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_43_44442_s_376	15304493	A cysteine residue that had been added to the beta-subunit COOH terminus of a bifunctional hCG analog ( i.e. CFC101 - 114,) S138Cthat binds LHR and FSHR was found to become cross-linked to cysteines  added to the alpha-subunit during heterodimer synthesis in COS-7 cells.	bind
41614	1	9867	7	11	NULL	NULL	NULL	hCG analog	GP		binds			S138C in the beta-subunit COOH terminus		LHR	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_43_44442_s_376	15304493	A cysteine residue that had been added to the beta-subunit COOH terminus of a bifunctional hCG analog ( i.e. CFC101 - 114,) S138Cthat binds LHR and FSHR was found to become cross-linked to cysteines  added to the alpha-subunit during heterodimer synthesis in COS-7 cells.	bind
41615	2	9867	7	11	NULL	NULL	NULL	hCG analog	GP		binds			S138C in the beta-subunit COOH terminus		FSHR	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_43_44442_s_376	15304493	A cysteine residue that had been added to the beta-subunit COOH terminus of a bifunctional hCG analog ( i.e. CFC101 - 114,) S138Cthat binds LHR and FSHR was found to become cross-linked to cysteines  added to the alpha-subunit during heterodimer synthesis in COS-7 cells.	bind
41622	3	9867	7	11	NULL	NULL	NULL				crosslinked to			S138C					cysteines in alpha-subunit		NULL	COS-7 cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_43_44442_s_376	15304493	A cysteine residue that had been added to the beta-subunit COOH terminus of a bifunctional hCG analog ( i.e. CFC101 - 114,) S138Cthat binds LHR and FSHR was found to become cross-linked to cysteines  added to the alpha-subunit during heterodimer synthesis in COS-7 cells.	bind
41624	4	9867	7	11	NULL	NULL	NULL				added to			cysteines					alpha-subunit		NULL	COS-7 cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_43_44442_s_376	15304493	A cysteine residue that had been added to the beta-subunit COOH terminus of a bifunctional hCG analog ( i.e. CFC101 - 114,) S138Cthat binds LHR and FSHR was found to become cross-linked to cysteines  added to the alpha-subunit during heterodimer synthesis in COS-7 cells.	bind
41626	5	9867	7	11	NULL	NULL	NULL	statement 4	Process		occurs during					heterodimer synthesis	Process				NULL	COS-7 cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_43_44442_s_376	15304493	A cysteine residue that had been added to the beta-subunit COOH terminus of a bifunctional hCG analog ( i.e. CFC101 - 114,) S138Cthat binds LHR and FSHR was found to become cross-linked to cysteines  added to the alpha-subunit during heterodimer synthesis in COS-7 cells.	bind
34378	1	9868	6	11	NULL	NULL	NULL	ADAM12	GP		bind			cysteine rich domain		syndecan	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_43_32929_s_282	16945929	A cysteine-rich domain of ADAM12 binds syndecan that promotes mesenchymal cell spreading through integrin beta1 ( ).	bind
34379	2	9868	6	11	NULL	NULL	NULL	statement 1	Process		promotes					mesenchymal cell	Cell	spreading of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_43_32929_s_282	16945929	A cysteine-rich domain of ADAM12 binds syndecan that promotes mesenchymal cell spreading through integrin beta1 ( ).	bind
34381	3	9868	6	11	NULL	NULL	NULL	statement 2	Process		occurs through					integrin beta1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_43_32929_s_282	16945929	A cysteine-rich domain of ADAM12 binds syndecan that promotes mesenchymal cell spreading through integrin beta1 ( ).	bind
41627	1	9868	7	11	NULL	NULL	NULL	ADAM12	GP		binds			cysteine-rich domain		 syndecan	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_43_32929_s_282	16945929	A cysteine-rich domain of ADAM12 binds syndecan that promotes mesenchymal cell spreading through integrin beta1 ( ).	bind
41628	2	9868	7	11	NULL	NULL	NULL	statement 1	Process		promotes					mesenchymal cell 	Cell	spreading of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_43_32929_s_282	16945929	A cysteine-rich domain of ADAM12 binds syndecan that promotes mesenchymal cell spreading through integrin beta1 ( ).	bind
41629	3	9868	7	11	NULL	NULL	NULL	statement 2	Process		occurs through					integrin beta1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_43_32929_s_282	16945929	A cysteine-rich domain of ADAM12 binds syndecan that promotes mesenchymal cell spreading through integrin beta1 ( ).	bind
34384	1	9869	6	11	NULL	NULL	NULL	IkappaB kinase	GP	cytokine responsive	activates					NF-kappaB	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5523_s_476	9710636	A cytokine-responsive IkappaB kinase that activates the transcription factor NF-kappaB.	bind
34385	2	9869	6	11	NULL	NULL	NULL	NF-kappaB	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5523_s_476	9710636	A cytokine-responsive IkappaB kinase that activates the transcription factor NF-kappaB.	bind
41630	1	9869	7	11	NULL	NULL	NULL	IkappaB kinase	GP	cytokine-responsive	activates					NF-kappaB	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5523_s_476	9710636	A cytokine-responsive IkappaB kinase that activates the transcription factor NF-kappaB.	bind
41631	2	9869	7	11	NULL	NULL	NULL	NF-kappaB	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5523_s_476	9710636	A cytokine-responsive IkappaB kinase that activates the transcription factor NF-kappaB.	bind
34394	1	9870	6	11	NULL	NULL	NULL	cytolysin	Chemical	Salmonella	is required for					survival	Process				NULL	macrophages	NULL	NULL	NULL	NULL	gw60_infectimmun_69_2_706_s_326	11159958	A cytolysin encoded by  Salmonella is required for survival within macrophages.	bind
41633	2	9870	7	11	NULL	NULL	NULL	cytolysin	Chemical	Salmonella	is required for					survival	Process				NULL	macrophages	NULL	NULL	NULL	NULL	gw60_infectimmun_69_2_706_s_326	11159958	A cytolysin encoded by  Salmonella is required for survival within macrophages.	bind
34395	1	9871	6	11	NULL	NULL	NULL	chaperonin	GP	cytoplasmic	catalyzes					beta-actin	GP	folding of 			NULL		NULL	NULL	NULL	NULL	gw60_cell_103_4_621_s_380	11106732	A cytoplasmic chaperonin that catalyzes beta-actin folding.	bind
41634	1	9871	7	11	NULL	NULL	NULL	chaperonin 	GP	cytoplasmic	catalyzes					beta-actin	GP	folding of			NULL		NULL	NULL	NULL	NULL	gw60_cell_103_4_621_s_380	11106732	A cytoplasmic chaperonin that catalyzes beta-actin folding.	bind
34396	1	9872	6	11	NULL	NULL	NULL	serine protein kinase	GP	cytoplasmic	bind					FANCA	GP				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_67_0_481_s_495	9759495	A cytoplasmic serine protein kinase binds and may regulate the Fanconi anemia protein FANCA.	bind
34397	2	9872	6	11	NULL	NULL	NULL	FANCA	GP		is					Fanconi anemia protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_67_0_481_s_495	9759495	A cytoplasmic serine protein kinase binds and may regulate the Fanconi anemia protein FANCA.	bind
34398	3	9872	6	11	NULL	NULL	NULL	statement 1	Process		regulates		may			FANCA	GP				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_67_0_481_s_495	9759495	A cytoplasmic serine protein kinase binds and may regulate the Fanconi anemia protein FANCA.	bind
41635	1	9872	7	11	NULL	NULL	NULL	serine protein kinase	GP	cytoplasmic	binds					FANCA protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_67_0_481_s_495	9759495	A cytoplasmic serine protein kinase binds and may regulate the Fanconi anemia protein FANCA.	bind
41636	2	9872	7	11	NULL	NULL	NULL	statement 1	Process		regulate		may			FANCA protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_67_0_481_s_495	9759495	A cytoplasmic serine protein kinase binds and may regulate the Fanconi anemia protein FANCA.	bind
41637	3	9872	7	11	NULL	NULL	NULL	FANCA	GP		is					Fanconi anemia	GP				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_67_0_481_s_495	9759495	A cytoplasmic serine protein kinase binds and may regulate the Fanconi anemia protein FANCA.	bind
34399	1	9873	6	11	NULL	NULL	NULL	tropomyosin	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2101_s_384	10595939	A cytoskeletal protein that binds to the end of erythrocyte tropomyosin and inhibits tropomyosin binding to actin.	bind
34400	2	9873	6	11	NULL	NULL	NULL	cytoskeletal protein	GP		bind					erythrocyte tropomyosin	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2101_s_384	10595939	A cytoskeletal protein that binds to the end of erythrocyte tropomyosin and inhibits tropomyosin binding to actin.	bind
34401	3	9873	6	11	NULL	NULL	NULL	statement 2	Process		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2101_s_384	10595939	A cytoskeletal protein that binds to the end of erythrocyte tropomyosin and inhibits tropomyosin binding to actin.	bind
41638	1	9873	7	11	NULL	NULL	NULL	cytoskeletal protein	GP		binds to					erythrocyte tropomyosin 	GP		end of		NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2101_s_384	10595939	A cytoskeletal protein that binds to the end of erythrocyte tropomyosin and inhibits tropomyosin binding to actin.	bind
41639	2	9873	7	11	NULL	NULL	NULL	tropomyosin	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2101_s_384	10595939	A cytoskeletal protein that binds to the end of erythrocyte tropomyosin and inhibits tropomyosin binding to actin.	bind
41640	3	9873	7	11	NULL	NULL	NULL	statement 1	Process		inhibits					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_155_6_2101_s_384	10595939	A cytoskeletal protein that binds to the end of erythrocyte tropomyosin and inhibits tropomyosin binding to actin.	bind
34691	1	9874	6	11	NULL	NULL	NULL	cytosolic PGES	GP		is					CPGES	GP				NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_73_1_36_s_25	15744024	A cytosolic PGES (CPGES), also known as cytosolic PTGES or PTGES3, identical to p23, a ubiquitous chaperone protein weakly bound to the steroid hormone receptor/hsp90 complex [ ,  ], was characterized and found coupled to COX1 for immediate production of PGE2 [ ].	bind
34698	2	9874	6	11	NULL	NULL	NULL	CPGES	GP		is coupled to					COX1	GP				NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_73_1_36_s_25	15744024	A cytosolic PGES (CPGES), also known as cytosolic PTGES or PTGES3, identical to p23, a ubiquitous chaperone protein weakly bound to the steroid hormone receptor/hsp90 complex [ ,  ], was characterized and found coupled to COX1 for immediate production of PGE2 [ ].	bind
34699	3	9874	6	11	NULL	NULL	NULL	statement 2	Process		leads to					PGE2	GP	production of			NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_73_1_36_s_25	15744024	A cytosolic PGES (CPGES), also known as cytosolic PTGES or PTGES3, identical to p23, a ubiquitous chaperone protein weakly bound to the steroid hormone receptor/hsp90 complex [ ,  ], was characterized and found coupled to COX1 for immediate production of PGE2 [ ].	bind
34700	4	9874	6	11	NULL	NULL	NULL	CPGES	GP		is identical to					p23	GP				NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_73_1_36_s_25	15744024	A cytosolic PGES (CPGES), also known as cytosolic PTGES or PTGES3, identical to p23, a ubiquitous chaperone protein weakly bound to the steroid hormone receptor/hsp90 complex [ ,  ], was characterized and found coupled to COX1 for immediate production of PGE2 [ ].	bind
48997	5	9874	6	11	NULL	NULL	NULL	CPGES	GP		is					PTGES3	GP				NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_73_1_36_s_25	15744024	A cytosolic PGES (CPGES), also known as cytosolic PTGES or PTGES3, identical to p23, a ubiquitous chaperone protein weakly bound to the steroid hormone receptor/hsp90 complex [ ,  ], was characterized and found coupled to COX1 for immediate production of PGE2 [ ].	bind
48998	6	9874	6	11	NULL	NULL	NULL	CPGES	GP		is					cytosolic PTGES	GP				NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_73_1_36_s_25	15744024	A cytosolic PGES (CPGES), also known as cytosolic PTGES or PTGES3, identical to p23, a ubiquitous chaperone protein weakly bound to the steroid hormone receptor/hsp90 complex [ ,  ], was characterized and found coupled to COX1 for immediate production of PGE2 [ ].	bind
48999	7	9874	6	11	NULL	NULL	NULL	p23	GP		is a type of					ubiquitous chaperone protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_73_1_36_s_25	15744024	A cytosolic PGES (CPGES), also known as cytosolic PTGES or PTGES3, identical to p23, a ubiquitous chaperone protein weakly bound to the steroid hormone receptor/hsp90 complex [ ,  ], was characterized and found coupled to COX1 for immediate production of PGE2 [ ].	bind
49000	8	9874	6	11	NULL	NULL	NULL	p23	GP		bind		weakly			steroid hormone receptor/hsp90 complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_73_1_36_s_25	15744024	A cytosolic PGES (CPGES), also known as cytosolic PTGES or PTGES3, identical to p23, a ubiquitous chaperone protein weakly bound to the steroid hormone receptor/hsp90 complex [ ,  ], was characterized and found coupled to COX1 for immediate production of PGE2 [ ].	bind
41641	1	9874	7	11	NULL	NULL	NULL	CPGES	GP		is					cytosolic PTGES	GP				NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_73_1_36_s_25	15744024	A cytosolic PGES (CPGES), also known as cytosolic PTGES or PTGES3, identical to p23, a ubiquitous chaperone protein weakly bound to the steroid hormone receptor/hsp90 complex [ ,  ], was characterized and found coupled to COX1 for immediate production of PGE2 [ ].	bind
41642	2	9874	7	11	NULL	NULL	NULL	CPGES	GP		is					PTGES3	GP				NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_73_1_36_s_25	15744024	A cytosolic PGES (CPGES), also known as cytosolic PTGES or PTGES3, identical to p23, a ubiquitous chaperone protein weakly bound to the steroid hormone receptor/hsp90 complex [ ,  ], was characterized and found coupled to COX1 for immediate production of PGE2 [ ].	bind
41643	3	9874	7	11	NULL	NULL	NULL	CPGES	GP		is identical to					p23	GP				NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_73_1_36_s_25	15744024	A cytosolic PGES (CPGES), also known as cytosolic PTGES or PTGES3, identical to p23, a ubiquitous chaperone protein weakly bound to the steroid hormone receptor/hsp90 complex [ ,  ], was characterized and found coupled to COX1 for immediate production of PGE2 [ ].	bind
41644	4	9874	7	11	NULL	NULL	NULL	CPGES	GP		is					cytosolic PGES	GP				NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_73_1_36_s_25	15744024	A cytosolic PGES (CPGES), also known as cytosolic PTGES or PTGES3, identical to p23, a ubiquitous chaperone protein weakly bound to the steroid hormone receptor/hsp90 complex [ ,  ], was characterized and found coupled to COX1 for immediate production of PGE2 [ ].	bind
41645	5	9874	7	11	NULL	NULL	NULL	p23	GP		is a type of					ubiquitous chaperone protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_73_1_36_s_25	15744024	A cytosolic PGES (CPGES), also known as cytosolic PTGES or PTGES3, identical to p23, a ubiquitous chaperone protein weakly bound to the steroid hormone receptor/hsp90 complex [ ,  ], was characterized and found coupled to COX1 for immediate production of PGE2 [ ].	bind
41646	6	9874	7	11	NULL	NULL	NULL	p23	GP		bind		weakly			steroid hormone receptor/hsp90 complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_73_1_36_s_25	15744024	A cytosolic PGES (CPGES), also known as cytosolic PTGES or PTGES3, identical to p23, a ubiquitous chaperone protein weakly bound to the steroid hormone receptor/hsp90 complex [ ,  ], was characterized and found coupled to COX1 for immediate production of PGE2 [ ].	bind
41647	7	9874	7	11	NULL	NULL	NULL	CPGES	GP		coupled to					COX1	GP				NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_73_1_36_s_25	15744024	A cytosolic PGES (CPGES), also known as cytosolic PTGES or PTGES3, identical to p23, a ubiquitous chaperone protein weakly bound to the steroid hormone receptor/hsp90 complex [ ,  ], was characterized and found coupled to COX1 for immediate production of PGE2 [ ].	bind
41648	8	9874	7	11	NULL	NULL	NULL	statement 7	Process		leads to					PGE2	GP	immediate production of			NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_73_1_36_s_25	15744024	A cytosolic PGES (CPGES), also known as cytosolic PTGES or PTGES3, identical to p23, a ubiquitous chaperone protein weakly bound to the steroid hormone receptor/hsp90 complex [ ,  ], was characterized and found coupled to COX1 for immediate production of PGE2 [ ].	bind
34402	1	9875	6	11	NULL	NULL	NULL	cytosolic protein factor	GP		bind		specifically			H-ferritin	GP			3''-UTR	NULL	THP-1 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_42_30209_s_6	10514512	A cytosolic protein factor from THP-1 cells was found to specifically bind to H-ferritin 3''-UTR.	bind
41649	1	9875	7	11	NULL	NULL	NULL	cytosolic protein factor	GP		bind		specifically			H-ferritin	GP			 3''-UTR	NULL	THP-1 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_42_30209_s_6	10514512	A cytosolic protein factor from THP-1 cells was found to specifically bind to H-ferritin 3''-UTR.	bind
34403	1	9876	6	11	NULL	NULL	NULL	cytotoxic mAb	GP		bind					ErbB-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_113_9_1307_s_342	15124022	A cytotoxic mAb that binds to ErbB-2, a member of the EGFR family, and induced apoptosis has been reported ( ).	bind
34404	2	9876	6	11	NULL	NULL	NULL	ErbB-2	GP		is a member of					EGFR family	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_113_9_1307_s_342	15124022	A cytotoxic mAb that binds to ErbB-2, a member of the EGFR family, and induced apoptosis has been reported ( ).	bind
49001	3	9876	6	11	NULL	NULL	NULL	statement 1	Process		induces					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_113_9_1307_s_342	15124022	A cytotoxic mAb that binds to ErbB-2, a member of the EGFR family, and induced apoptosis has been reported ( ).	bind
41650	1	9876	7	11	NULL	NULL	NULL	cytotoxic mAb	GP		binds to					ErbB-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_113_9_1307_s_342	15124022	A cytotoxic mAb that binds to ErbB-2, a member of the EGFR family, and induced apoptosis has been reported ( ).	bind
41651	2	9876	7	11	NULL	NULL	NULL	statement 1	Process		induce					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_113_9_1307_s_342	15124022	A cytotoxic mAb that binds to ErbB-2, a member of the EGFR family, and induced apoptosis has been reported ( ).	bind
41652	3	9876	7	11	NULL	NULL	NULL	ErbB-2	GP		is a member of					EGFR family	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_113_9_1307_s_342	15124022	A cytotoxic mAb that binds to ErbB-2, a member of the EGFR family, and induced apoptosis has been reported ( ).	bind
34405	1	9877	6	11	NULL	NULL	NULL	SEB	GP		bind					Daudi cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_immunity_5_2_137_s_73	8769477	A cytotoxicity assay was used to determine whether 1B2 Fab fragments could inhibit the 2C-mediated recognition of SEB, SEC1, and SEC3 bound to Daudi cells.	bind
34406	2	9877	6	11	NULL	NULL	NULL	SEC1	GP		bind					Daudi cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_immunity_5_2_137_s_73	8769477	A cytotoxicity assay was used to determine whether 1B2 Fab fragments could inhibit the 2C-mediated recognition of SEB, SEC1, and SEC3 bound to Daudi cells.	bind
34407	3	9877	6	11	NULL	NULL	NULL	SEC3	GP		bind					Daudi cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_immunity_5_2_137_s_73	8769477	A cytotoxicity assay was used to determine whether 1B2 Fab fragments could inhibit the 2C-mediated recognition of SEB, SEC1, and SEC3 bound to Daudi cells.	bind
41653	1	9877	7	11	NULL	NULL	NULL	SEB	GP		bind					Daudi cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_immunity_5_2_137_s_73	8769477	A cytotoxicity assay was used to determine whether 1B2 Fab fragments could inhibit the 2C-mediated recognition of SEB, SEC1, and SEC3 bound to Daudi cells.	bind
41654	2	9877	7	11	NULL	NULL	NULL	SEC1	GP		bind					Daudi cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_immunity_5_2_137_s_73	8769477	A cytotoxicity assay was used to determine whether 1B2 Fab fragments could inhibit the 2C-mediated recognition of SEB, SEC1, and SEC3 bound to Daudi cells.	bind
41655	3	9877	7	11	NULL	NULL	NULL	SEC3	Cell		bind					Daudi cells	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_5_2_137_s_73	8769477	A cytotoxicity assay was used to determine whether 1B2 Fab fragments could inhibit the 2C-mediated recognition of SEB, SEC1, and SEC3 bound to Daudi cells.	bind
34642	1	9878	6	11	NULL	NULL	NULL	D1 receptor	GP		does not bind			S198A		dopamine	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_44_37225_s_190	16115864	A D1 receptor generated with two of these serines, Ser198 and Ser199, substituted with alanine (D1(S198A/S199A)) did not bind dopamine or SCH 23390, but we determined that it did bind (+)BTC.	bind
34643	2	9878	6	11	NULL	NULL	NULL	D1 receptor	GP		does not bind			S199A		dopamine	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_44_37225_s_190	16115864	A D1 receptor generated with two of these serines, Ser198 and Ser199, substituted with alanine (D1(S198A/S199A)) did not bind dopamine or SCH 23390, but we determined that it did bind (+)BTC.	bind
34644	3	9878	6	11	NULL	NULL	NULL	D1 receptor	GP		does not bind			S198A		SCH 23390	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_44_37225_s_190	16115864	A D1 receptor generated with two of these serines, Ser198 and Ser199, substituted with alanine (D1(S198A/S199A)) did not bind dopamine or SCH 23390, but we determined that it did bind (+)BTC.	bind
34645	4	9878	6	11	NULL	NULL	NULL	D1 receptor	GP		does not bind			S199A		SCH 23390	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_44_37225_s_190	16115864	A D1 receptor generated with two of these serines, Ser198 and Ser199, substituted with alanine (D1(S198A/S199A)) did not bind dopamine or SCH 23390, but we determined that it did bind (+)BTC.	bind
34646	5	9878	6	11	NULL	NULL	NULL	D1 receptor	GP		bind			S198A		BTC	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_44_37225_s_190	16115864	A D1 receptor generated with two of these serines, Ser198 and Ser199, substituted with alanine (D1(S198A/S199A)) did not bind dopamine or SCH 23390, but we determined that it did bind (+)BTC.	bind
34647	6	9878	6	11	NULL	NULL	NULL	D1 receptor	GP		bind			S199A		BTC	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_44_37225_s_190	16115864	A D1 receptor generated with two of these serines, Ser198 and Ser199, substituted with alanine (D1(S198A/S199A)) did not bind dopamine or SCH 23390, but we determined that it did bind (+)BTC.	bind
34648	7	9878	6	11	NULL	NULL	NULL	S198A	AminoAcid		is					serine198 substituted with alanine	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_44_37225_s_190	16115864	A D1 receptor generated with two of these serines, Ser198 and Ser199, substituted with alanine (D1(S198A/S199A)) did not bind dopamine or SCH 23390, but we determined that it did bind (+)BTC.	bind
34690	8	9878	6	11	NULL	NULL	NULL	S199A	AminoAcid		is					serine199 substituted with alanine	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_44_37225_s_190	16115864	A D1 receptor generated with two of these serines, Ser198 and Ser199, substituted with alanine (D1(S198A/S199A)) did not bind dopamine or SCH 23390, but we determined that it did bind (+)BTC.	bind
41659	1	9878	7	11	NULL	NULL	NULL	D1 receptor	GP		does not bind			S198A/S199A		dopamine	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_44_37225_s_190	16115864	A D1 receptor generated with two of these serines, Ser198 and Ser199, substituted with alanine (D1(S198A/S199A)) did not bind dopamine or SCH 23390, but we determined that it did bind (+)BTC.	bind
41660	2	9878	7	11	NULL	NULL	NULL	D1 receptor	GP		does not bind			S198A/S199A		SCH 23390	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_44_37225_s_190	16115864	A D1 receptor generated with two of these serines, Ser198 and Ser199, substituted with alanine (D1(S198A/S199A)) did not bind dopamine or SCH 23390, but we determined that it did bind (+)BTC.	bind
41661	3	9878	7	11	NULL	NULL	NULL	D1 receptor	GP		bind			S198A/S199A		BTC	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_44_37225_s_190	16115864	A D1 receptor generated with two of these serines, Ser198 and Ser199, substituted with alanine (D1(S198A/S199A)) did not bind dopamine or SCH 23390, but we determined that it did bind (+)BTC.	bind
49548	4	9878	7	11	NULL	NULL	NULL	S198A	AminoAcid		is					serine198 substituted with alanine	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_44_37225_s_190	16115864	A D1 receptor generated with two of these serines, Ser198 and Ser199, substituted with alanine (D1(S198A/S199A)) did not bind dopamine or SCH 23390, but we determined that it did bind (+)BTC.	bind
49549	5	9878	7	11	NULL	NULL	NULL	S199A	AminoAcid		is					serine199 substituted with alanine	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_44_37225_s_190	16115864	A D1 receptor generated with two of these serines, Ser198 and Ser199, substituted with alanine (D1(S198A/S199A)) did not bind dopamine or SCH 23390, but we determined that it did bind (+)BTC.	bind
34408	1	9879	6	11	NULL	NULL	NULL	FYB	GP		bind					FYN	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbpathogenesis_27_4_231_s_116	10502464	A Da Silva, Z Li, C De Vera, E Canto, P Findell and CE Rudd, Cloning of a novel  T-cell protein FYB that binds FYN and SH2-domain-containing leukocyte protein 76  and modulates interleukin 2 production.	bind
34409	2	9879	6	11	NULL	NULL	NULL	leukocyte protein 76	GP		contains								SH2 domain		NULL		NULL	NULL	NULL	NULL	gw70_microbpathogenesis_27_4_231_s_116	10502464	A Da Silva, Z Li, C De Vera, E Canto, P Findell and CE Rudd, Cloning of a novel  T-cell protein FYB that binds FYN and SH2-domain-containing leukocyte protein 76  and modulates interleukin 2 production.	bind
34410	3	9879	6	11	NULL	NULL	NULL	statement 5	Process		modulates					interleukin 2	GP	production of			NULL		NULL	NULL	NULL	NULL	gw70_microbpathogenesis_27_4_231_s_116	10502464	A Da Silva, Z Li, C De Vera, E Canto, P Findell and CE Rudd, Cloning of a novel  T-cell protein FYB that binds FYN and SH2-domain-containing leukocyte protein 76  and modulates interleukin 2 production.	bind
49002	4	9879	6	11	NULL	NULL	NULL	FYB	GP		is a type of					novel T-cell protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbpathogenesis_27_4_231_s_116	10502464	A Da Silva, Z Li, C De Vera, E Canto, P Findell and CE Rudd, Cloning of a novel  T-cell protein FYB that binds FYN and SH2-domain-containing leukocyte protein 76  and modulates interleukin 2 production.	bind
49532	5	9879	6	11	NULL	NULL	NULL	FYB	GP		bind					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbpathogenesis_27_4_231_s_116	10502464	A Da Silva, Z Li, C De Vera, E Canto, P Findell and CE Rudd, Cloning of a novel  T-cell protein FYB that binds FYN and SH2-domain-containing leukocyte protein 76  and modulates interleukin 2 production.	bind
41662	1	9879	7	11	NULL	NULL	NULL	FYB	GP		binds					FYN	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbpathogenesis_27_4_231_s_116	10502464	A Da Silva, Z Li, C De Vera, E Canto, P Findell and CE Rudd, Cloning of a novel  T-cell protein FYB that binds FYN and SH2-domain-containing leukocyte protein 76  and modulates interleukin 2 production.	bind
41663	5	9879	7	11	NULL	NULL	NULL	FYB	GP		binds					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbpathogenesis_27_4_231_s_116	10502464	A Da Silva, Z Li, C De Vera, E Canto, P Findell and CE Rudd, Cloning of a novel  T-cell protein FYB that binds FYN and SH2-domain-containing leukocyte protein 76  and modulates interleukin 2 production.	bind
41664	3	9879	7	11	NULL	NULL	NULL	FYB	GP		modulates					interleukin 2	GP	production of			NULL		NULL	NULL	NULL	NULL	gw70_microbpathogenesis_27_4_231_s_116	10502464	A Da Silva, Z Li, C De Vera, E Canto, P Findell and CE Rudd, Cloning of a novel  T-cell protein FYB that binds FYN and SH2-domain-containing leukocyte protein 76  and modulates interleukin 2 production.	bind
41665	4	9879	7	11	NULL	NULL	NULL	FYB	GP		is a type of					novel T-cell protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbpathogenesis_27_4_231_s_116	10502464	A Da Silva, Z Li, C De Vera, E Canto, P Findell and CE Rudd, Cloning of a novel  T-cell protein FYB that binds FYN and SH2-domain-containing leukocyte protein 76  and modulates interleukin 2 production.	bind
49533	2	9879	7	11	NULL	NULL	NULL	 leukocyte protein 76	GP		contains								SH2 domain		NULL		NULL	NULL	NULL	NULL	gw70_microbpathogenesis_27_4_231_s_116	10502464	A Da Silva, Z Li, C De Vera, E Canto, P Findell and CE Rudd, Cloning of a novel  T-cell protein FYB that binds FYN and SH2-domain-containing leukocyte protein 76  and modulates interleukin 2 production.	bind
34635	1	9880	6	11	NULL	NULL	NULL	Daam1	GP		bind			C-terminal fragment		Dsh	GP		PDZ domain		NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_21_0_155_s_198	16212491	A Daam1 C-terminal fragment binds the Dsh PDZ and DEP domains, the N-terminal part  of Daam1 binds RhoA, and Daam1 is required for Fz-mediated Rho activation in  Xenopus ( Habas et al. 2001), which makes Daam1 a good candidate to recruit Rho to the sites of Dsh localization.	bind
34636	2	9880	6	11	NULL	NULL	NULL	Daam1	GP		bind			C-terminal fragment		Dsh	GP		DEP domain		NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_21_0_155_s_198	16212491	A Daam1 C-terminal fragment binds the Dsh PDZ and DEP domains, the N-terminal part  of Daam1 binds RhoA, and Daam1 is required for Fz-mediated Rho activation in  Xenopus ( Habas et al. 2001), which makes Daam1 a good candidate to recruit Rho to the sites of Dsh localization.	bind
34637	3	9880	6	11	NULL	NULL	NULL	Daam1	GP		bind			N-terminal part		RhoA	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_21_0_155_s_198	16212491	A Daam1 C-terminal fragment binds the Dsh PDZ and DEP domains, the N-terminal part  of Daam1 binds RhoA, and Daam1 is required for Fz-mediated Rho activation in  Xenopus ( Habas et al. 2001), which makes Daam1 a good candidate to recruit Rho to the sites of Dsh localization.	bind
34638	4	9880	6	11	NULL	NULL	NULL	Rho	GP	activation of	is mediated by					Fz	GP				NULL	Xenopus	NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_21_0_155_s_198	16212491	A Daam1 C-terminal fragment binds the Dsh PDZ and DEP domains, the N-terminal part  of Daam1 binds RhoA, and Daam1 is required for Fz-mediated Rho activation in  Xenopus ( Habas et al. 2001), which makes Daam1 a good candidate to recruit Rho to the sites of Dsh localization.	bind
34639	5	9880	6	11	NULL	NULL	NULL	Daam1	GP		is required for					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_21_0_155_s_198	16212491	A Daam1 C-terminal fragment binds the Dsh PDZ and DEP domains, the N-terminal part  of Daam1 binds RhoA, and Daam1 is required for Fz-mediated Rho activation in  Xenopus ( Habas et al. 2001), which makes Daam1 a good candidate to recruit Rho to the sites of Dsh localization.	bind
34640	6	9880	6	11	NULL	NULL	NULL	Rho	GP		is recruited to					Dsh localization	GP	sites of 			NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_21_0_155_s_198	16212491	A Daam1 C-terminal fragment binds the Dsh PDZ and DEP domains, the N-terminal part  of Daam1 binds RhoA, and Daam1 is required for Fz-mediated Rho activation in  Xenopus ( Habas et al. 2001), which makes Daam1 a good candidate to recruit Rho to the sites of Dsh localization.	bind
34641	7	9880	6	11	NULL	NULL	NULL	Daam1	GP		plays a role in					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_21_0_155_s_198	16212491	A Daam1 C-terminal fragment binds the Dsh PDZ and DEP domains, the N-terminal part  of Daam1 binds RhoA, and Daam1 is required for Fz-mediated Rho activation in  Xenopus ( Habas et al. 2001), which makes Daam1 a good candidate to recruit Rho to the sites of Dsh localization.	bind
41666	1	9880	7	11	NULL	NULL	NULL	Daam1	GP		binds			C-terminal fragment		Dsh	GP		 PDZ domain		NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_21_0_155_s_198	16212491	A Daam1 C-terminal fragment binds the Dsh PDZ and DEP domains, the N-terminal part  of Daam1 binds RhoA, and Daam1 is required for Fz-mediated Rho activation in  Xenopus ( Habas et al. 2001), which makes Daam1 a good candidate to recruit Rho to the sites of Dsh localization.	bind
41667	2	9880	7	11	NULL	NULL	NULL	Daam1	GP		binds			C-terminal fragment		Dsh	GP		DEP domain		NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_21_0_155_s_198	16212491	A Daam1 C-terminal fragment binds the Dsh PDZ and DEP domains, the N-terminal part  of Daam1 binds RhoA, and Daam1 is required for Fz-mediated Rho activation in  Xenopus ( Habas et al. 2001), which makes Daam1 a good candidate to recruit Rho to the sites of Dsh localization.	bind
41668	3	9880	7	11	NULL	NULL	NULL	Daam1	GP		binds			N-terminal part		RhoA	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_21_0_155_s_198	16212491	A Daam1 C-terminal fragment binds the Dsh PDZ and DEP domains, the N-terminal part  of Daam1 binds RhoA, and Daam1 is required for Fz-mediated Rho activation in  Xenopus ( Habas et al. 2001), which makes Daam1 a good candidate to recruit Rho to the sites of Dsh localization.	bind
41669	4	9880	7	11	NULL	NULL	NULL	Fz	GP		mediates					Rho	GP	activation of			NULL	Xenopus	NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_21_0_155_s_198	16212491	A Daam1 C-terminal fragment binds the Dsh PDZ and DEP domains, the N-terminal part  of Daam1 binds RhoA, and Daam1 is required for Fz-mediated Rho activation in  Xenopus ( Habas et al. 2001), which makes Daam1 a good candidate to recruit Rho to the sites of Dsh localization.	bind
41671	5	9880	7	11	NULL	NULL	NULL	Daam1	GP		is required for					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_21_0_155_s_198	16212491	A Daam1 C-terminal fragment binds the Dsh PDZ and DEP domains, the N-terminal part  of Daam1 binds RhoA, and Daam1 is required for Fz-mediated Rho activation in  Xenopus ( Habas et al. 2001), which makes Daam1 a good candidate to recruit Rho to the sites of Dsh localization.	bind
41672	6	9880	7	11	NULL	NULL	NULL	Daam1	GP		recruit					Rho	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_21_0_155_s_198	16212491	A Daam1 C-terminal fragment binds the Dsh PDZ and DEP domains, the N-terminal part  of Daam1 binds RhoA, and Daam1 is required for Fz-mediated Rho activation in  Xenopus ( Habas et al. 2001), which makes Daam1 a good candidate to recruit Rho to the sites of Dsh localization.	bind
41673	7	9880	7	11	NULL	NULL	NULL	statement 6	Process		occur at					Dsh localization	GP	sites of			NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_21_0_155_s_198	16212491	A Daam1 C-terminal fragment binds the Dsh PDZ and DEP domains, the N-terminal part  of Daam1 binds RhoA, and Daam1 is required for Fz-mediated Rho activation in  Xenopus ( Habas et al. 2001), which makes Daam1 a good candidate to recruit Rho to the sites of Dsh localization.	bind
34411	1	9882	6	11	NULL	NULL	NULL	lectin	Chemical	peroxidase-labeled;;peanut	bind		specifically			distal tubule cells	Cell	human			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_in-vitro-cell-dev-biol_26_5_2161826_s_8	2161826	A dark-brown reaction  product was observed in these cells when stained by the immunoperoxidase  method with peroxidase-labeled peanut lectin (Arachis hypogaea), which  binds specifically to human distal tubule and collecting duct cells.	bind
34412	2	9882	6	11	NULL	NULL	NULL	lectin	Chemical	peroxidase-labeled;;peanut	is					Arachis hypogaea	Organism				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_in-vitro-cell-dev-biol_26_5_2161826_s_8	2161826	A dark-brown reaction  product was observed in these cells when stained by the immunoperoxidase  method with peroxidase-labeled peanut lectin (Arachis hypogaea), which  binds specifically to human distal tubule and collecting duct cells.	bind
34492	3	9882	6	11	NULL	NULL	NULL	lectin	Chemical	peroxidase-labeled;;peanut	bind		specifically			collecting duct cells	Cell	human			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_in-vitro-cell-dev-biol_26_5_2161826_s_8	2161826	A dark-brown reaction  product was observed in these cells when stained by the immunoperoxidase  method with peroxidase-labeled peanut lectin (Arachis hypogaea), which  binds specifically to human distal tubule and collecting duct cells.	bind
41720	1	9882	7	11	NULL	NULL	NULL	lectin	Chemical	peroxidase-labeled;;peanut	bind		specifically			distal tubule	Cell	human			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_in-vitro-cell-dev-biol_26_5_2161826_s_8	2161826	A dark-brown reaction  product was observed in these cells when stained by the immunoperoxidase  method with peroxidase-labeled peanut lectin (Arachis hypogaea), which  binds specifically to human distal tubule and collecting duct cells.	bind
41721	2	9882	7	11	NULL	NULL	NULL	lectin	Chemical	peroxidase-labeled;;peanut	bind		specifically			collecting duct cells	Cell	human			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_in-vitro-cell-dev-biol_26_5_2161826_s_8	2161826	A dark-brown reaction  product was observed in these cells when stained by the immunoperoxidase  method with peroxidase-labeled peanut lectin (Arachis hypogaea), which  binds specifically to human distal tubule and collecting duct cells.	bind
41723	3	9882	7	11	NULL	NULL	NULL	lectin	Chemical	peroxidase-labeled;;peanut	is					Arachis hypogaea	Organism				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_in-vitro-cell-dev-biol_26_5_2161826_s_8	2161826	A dark-brown reaction  product was observed in these cells when stained by the immunoperoxidase  method with peroxidase-labeled peanut lectin (Arachis hypogaea), which  binds specifically to human distal tubule and collecting duct cells.	bind
34493	1	9884	6	11	NULL	NULL	NULL	RTP	GP		is					replication terminator protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_nature_430_7002_913_s_49	15286659	A database search revealed that tCdt1 most closely resembles bacterial replication  terminator protein (RTP), which binds to bacterial replicative helicase, DnaB 21.	bind
34494	2	9884	6	11	NULL	NULL	NULL	tCdt1	GP		resembles					RTP	GP	bacterial			NULL		NULL	NULL	NULL	NULL	gw70_nature_430_7002_913_s_49	15286659	A database search revealed that tCdt1 most closely resembles bacterial replication  terminator protein (RTP), which binds to bacterial replicative helicase, DnaB 21.	bind
34495	3	9884	6	11	NULL	NULL	NULL	DnaB	GP		is a type of					replicative helicase	GP				NULL		NULL	NULL	NULL	NULL	gw70_nature_430_7002_913_s_49	15286659	A database search revealed that tCdt1 most closely resembles bacterial replication  terminator protein (RTP), which binds to bacterial replicative helicase, DnaB 21.	bind
34496	4	9884	6	11	NULL	NULL	NULL	RTP	GP	bacterial	bind					DnaB	GP	bacterial			NULL		NULL	NULL	NULL	NULL	gw70_nature_430_7002_913_s_49	15286659	A database search revealed that tCdt1 most closely resembles bacterial replication  terminator protein (RTP), which binds to bacterial replicative helicase, DnaB 21.	bind
41732	1	9884	7	11	NULL	NULL	NULL	RTP	GP	bacterial	binds to					DnaB	GP	bacterial			NULL		NULL	NULL	NULL	NULL	gw70_nature_430_7002_913_s_49	15286659	A database search revealed that tCdt1 most closely resembles bacterial replication  terminator protein (RTP), which binds to bacterial replicative helicase, DnaB 21.	bind
41733	2	9884	7	11	NULL	NULL	NULL	RTP	GP		is					replication terminator protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_nature_430_7002_913_s_49	15286659	A database search revealed that tCdt1 most closely resembles bacterial replication  terminator protein (RTP), which binds to bacterial replicative helicase, DnaB 21.	bind
41734	3	9884	7	11	NULL	NULL	NULL	DnaB	GP		is a type of					replicative helicase	GP				NULL		NULL	NULL	NULL	NULL	gw70_nature_430_7002_913_s_49	15286659	A database search revealed that tCdt1 most closely resembles bacterial replication  terminator protein (RTP), which binds to bacterial replicative helicase, DnaB 21.	bind
41735	4	9884	7	11	NULL	NULL	NULL	tCdt1	GP		resembles					RTP	GP	bacterial			NULL		NULL	NULL	NULL	NULL	gw70_nature_430_7002_913_s_49	15286659	A database search revealed that tCdt1 most closely resembles bacterial replication  terminator protein (RTP), which binds to bacterial replicative helicase, DnaB 21.	bind
34497	1	9885	6	11	NULL	NULL	NULL	DBE probe	GP	mutant	does not bind				YY1 core recognition sequence	GST-YY1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_110_3_339_s_131	12176321	A DBE probe containing a mutation within the YY1 core recognition sequence was not bound by GST-YY1.	bind
41736	1	9885	7	11	NULL	NULL	NULL	DBE probe	GP	mutant	does not bind			 	YY1 core recognition sequence	GST-YY1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_110_3_339_s_131	12176321	A DBE probe containing a mutation within the YY1 core recognition sequence was not bound by GST-YY1.	bind
34498	1	9886	6	11	NULL	NULL	NULL	MCP	GP		is present on					spermatozoa	Cell	acrosome-reacted; human			NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_71_4_1374_s_299	15215199	A decade ago, Anderson and colleagues [ ] demonstrated that MCP on acrosome-reacted human spermatozoa specifically bound dimeric C3b and implicated this association in the adhesion of sperm and oocyte.	bind
34499	2	9886	6	11	NULL	NULL	NULL	MCP	GP		bind		specifically			dimeric C3b	GP				NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_71_4_1374_s_299	15215199	A decade ago, Anderson and colleagues [ ] demonstrated that MCP on acrosome-reacted human spermatozoa specifically bound dimeric C3b and implicated this association in the adhesion of sperm and oocyte.	bind
34500	3	9886	6	11	NULL	NULL	NULL	statement 2	Process		plays a role in					sperm	Cell	adhesion of 			NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_71_4_1374_s_299	15215199	A decade ago, Anderson and colleagues [ ] demonstrated that MCP on acrosome-reacted human spermatozoa specifically bound dimeric C3b and implicated this association in the adhesion of sperm and oocyte.	bind
34501	4	9886	6	11	NULL	NULL	NULL	statement 2	Process		plays a role in					oocyte	Cell	adhesion of			NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_71_4_1374_s_299	15215199	A decade ago, Anderson and colleagues [ ] demonstrated that MCP on acrosome-reacted human spermatozoa specifically bound dimeric C3b and implicated this association in the adhesion of sperm and oocyte.	bind
41756	1	9886	7	11	NULL	NULL	NULL	 MCP	GP		bind		specifically			dimeric C3b	GP				NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_71_4_1374_s_299	15215199	A decade ago, Anderson and colleagues [ ] demonstrated that MCP on acrosome-reacted human spermatozoa specifically bound dimeric C3b and implicated this association in the adhesion of sperm and oocyte.	bind
41759	2	9886	7	11	NULL	NULL	NULL	statement 1	Process		plays a role in					sperm	Cell	adhesion of			NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_71_4_1374_s_299	15215199	A decade ago, Anderson and colleagues [ ] demonstrated that MCP on acrosome-reacted human spermatozoa specifically bound dimeric C3b and implicated this association in the adhesion of sperm and oocyte.	bind
41784	3	9886	7	11	NULL	NULL	NULL	statement 1	Process		plays a role in					oocyte	Cell	adhesion of			NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_71_4_1374_s_299	15215199	A decade ago, Anderson and colleagues [ ] demonstrated that MCP on acrosome-reacted human spermatozoa specifically bound dimeric C3b and implicated this association in the adhesion of sperm and oocyte.	bind
49003	4	9886	7	11	NULL	NULL	NULL	MCP	GP		is present on					spermatozoa	Cell	acrosome-reacted;;human			NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_71_4_1374_s_299	15215199	A decade ago, Anderson and colleagues [ ] demonstrated that MCP on acrosome-reacted human spermatozoa specifically bound dimeric C3b and implicated this association in the adhesion of sperm and oocyte.	bind
41790	1	9887	7	NULL	NULL	0	NULL	HUVEC	NULL		produce	NULL				 essential complement factors	NULL				NULL		0	NULL	NULL	NULL	gw70_femsimmunolmedmic_36_1_55_s_146	12727366	A decade ago, we demonstrated that HUVEC produce the essential complement factors  for the binding of C3b and the terminal complement complex to co-cultured particulate  complement activators of the alternative pathway like agarose beads [  32].	bind
41793	2	9887	7	NULL	NULL	0	NULL	statement 1	NULL		is required for	NULL				C3b	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw70_femsimmunolmedmic_36_1_55_s_146	12727366	A decade ago, we demonstrated that HUVEC produce the essential complement factors  for the binding of C3b and the terminal complement complex to co-cultured particulate  complement activators of the alternative pathway like agarose beads [  32].	bind
41797	3	9887	7	NULL	NULL	0	NULL	HUVEC	NULL		produce	NULL				terminal complement complex	NULL				NULL		0	NULL	NULL	NULL	gw70_femsimmunolmedmic_36_1_55_s_146	12727366	A decade ago, we demonstrated that HUVEC produce the essential complement factors  for the binding of C3b and the terminal complement complex to co-cultured particulate  complement activators of the alternative pathway like agarose beads [  32].	bind
34503	1	9888	6	11	NULL	NULL	NULL	Cu	Chemical		bind					apo-CuZnSOD	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_annurevnutr_20_0_291_s_136	10940336	A decline in GSH levels in a cell impairs the subsequent binding of Cu to apo-CuZnSOD  ( 126) or the delivery of Cu to the cytosolic enzymes ( 119).	bind
34504	2	9888	6	11	NULL	NULL	NULL	GSH levels	GP	decline of	impairs					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevnutr_20_0_291_s_136	10940336	A decline in GSH levels in a cell impairs the subsequent binding of Cu to apo-CuZnSOD  ( 126) or the delivery of Cu to the cytosolic enzymes ( 119).	bind
34505	3	9888	6	11	NULL	NULL	NULL	Cu	Chemical		is delivered to					cytosolic enzymes	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevnutr_20_0_291_s_136	10940336	A decline in GSH levels in a cell impairs the subsequent binding of Cu to apo-CuZnSOD  ( 126) or the delivery of Cu to the cytosolic enzymes ( 119).	bind
34506	4	9888	6	11	NULL	NULL	NULL	GSH levels	GP	decline of	impairs					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevnutr_20_0_291_s_136	10940336	A decline in GSH levels in a cell impairs the subsequent binding of Cu to apo-CuZnSOD  ( 126) or the delivery of Cu to the cytosolic enzymes ( 119).	bind
41802	1	9888	7	11	NULL	NULL	NULL	Cu	Chemical		bind					apo-CuZnSOD	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_annurevnutr_20_0_291_s_136	10940336	A decline in GSH levels in a cell impairs the subsequent binding of Cu to apo-CuZnSOD  ( 126) or the delivery of Cu to the cytosolic enzymes ( 119).	bind
41803	2	9888	7	11	NULL	NULL	NULL	Cu	Chemical		delivered to					cytosolic enzymes	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevnutr_20_0_291_s_136	10940336	A decline in GSH levels in a cell impairs the subsequent binding of Cu to apo-CuZnSOD  ( 126) or the delivery of Cu to the cytosolic enzymes ( 119).	bind
41805	3	9888	7	11	NULL	NULL	NULL	GSH levels	GP	decline in	impairs					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevnutr_20_0_291_s_136	10940336	A decline in GSH levels in a cell impairs the subsequent binding of Cu to apo-CuZnSOD  ( 126) or the delivery of Cu to the cytosolic enzymes ( 119).	bind
41808	4	9888	7	11	NULL	NULL	NULL	GSH levels	GP	decline in	impairs 					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevnutr_20_0_291_s_136	10940336	A decline in GSH levels in a cell impairs the subsequent binding of Cu to apo-CuZnSOD  ( 126) or the delivery of Cu to the cytosolic enzymes ( 119).	bind
34633	1	9889	6	11	NULL	NULL	NULL	hamartin	GP	protein levels of	is decreased in					myrAkt cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_14_12361_s_69	12517744	A decline in the protein levels of the tuberin binding partner hamartin was also observed in myrAkt cells, and this decline was consistently accompanied by the appearance of a faster migrating species in hamartin immunoblots, suggesting the generation of a hamartin degradation product in cells with activated Akt.	bind
34634	2	9889	6	11	NULL	NULL	NULL	hamartin	GP		bind					tuberin	GP				NULL	myrAkt cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_278_14_12361_s_69	12517744	A decline in the protein levels of the tuberin binding partner hamartin was also observed in myrAkt cells, and this decline was consistently accompanied by the appearance of a faster migrating species in hamartin immunoblots, suggesting the generation of a hamartin degradation product in cells with activated Akt.	bind
41809	1	9889	7	11	NULL	NULL	NULL	hamartin	GP		bind					tuberin	GP				NULL	myrAkt cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_278_14_12361_s_69	12517744	A decline in the protein levels of the tuberin binding partner hamartin was also observed in myrAkt cells, and this decline was consistently accompanied by the appearance of a faster migrating species in hamartin immunoblots, suggesting the generation of a hamartin degradation product in cells with activated Akt.	bind
41810	2	9889	7	11	NULL	NULL	NULL	hamartin	GP	protein levels of	is decreased in					myrAkt cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_14_12361_s_69	12517744	A decline in the protein levels of the tuberin binding partner hamartin was also observed in myrAkt cells, and this decline was consistently accompanied by the appearance of a faster migrating species in hamartin immunoblots, suggesting the generation of a hamartin degradation product in cells with activated Akt.	bind
34630	1	9890	6	11	NULL	NULL	NULL	GCN4 gamma1 chimera	GP		folds into					homotypic coiled-coil dimers	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_23_6762_s_205	10581249	A decrease in binding affinity of the recombinant gamma1 chains and the chimeric GCN4 fusion proteins compared with native laminin-1 may be explained in terms of different coiled-coil structures in these molecules: the GCN4 gamma1 chimera folds into homotypic coiled-coil dimers and the gamma1 deltaN95AE fragments into a mixture of different oligomers, whereas the coiled-coil domain of native laminin-1 is a heterotrimer composed of alpha1, beta1 and gamma1 chains.	bind
34631	2	9890	6	11	NULL	NULL	NULL				folds into			gamma1 deltaN95AE fragments		oligomers	Chemical	mixture of different			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_23_6762_s_205	10581249	A decrease in binding affinity of the recombinant gamma1 chains and the chimeric GCN4 fusion proteins compared with native laminin-1 may be explained in terms of different coiled-coil structures in these molecules: the GCN4 gamma1 chimera folds into homotypic coiled-coil dimers and the gamma1 deltaN95AE fragments into a mixture of different oligomers, whereas the coiled-coil domain of native laminin-1 is a heterotrimer composed of alpha1, beta1 and gamma1 chains.	bind
34632	3	9890	6	11	NULL	NULL	NULL	laminin-1 	GP	native	is composed of			coiled coil domain					alpha1;; beta1;; gamma1		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_23_6762_s_205	10581249	A decrease in binding affinity of the recombinant gamma1 chains and the chimeric GCN4 fusion proteins compared with native laminin-1 may be explained in terms of different coiled-coil structures in these molecules: the GCN4 gamma1 chimera folds into homotypic coiled-coil dimers and the gamma1 deltaN95AE fragments into a mixture of different oligomers, whereas the coiled-coil domain of native laminin-1 is a heterotrimer composed of alpha1, beta1 and gamma1 chains.	bind
41811	1	9890	7	11	NULL	NULL	NULL	GCN4 gamma1 chimera 	GP		folds into					 homotypic coiled-coil dimers	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_23_6762_s_205	10581249	A decrease in binding affinity of the recombinant gamma1 chains and the chimeric GCN4 fusion proteins compared with native laminin-1 may be explained in terms of different coiled-coil structures in these molecules: the GCN4 gamma1 chimera folds into homotypic coiled-coil dimers and the gamma1 deltaN95AE fragments into a mixture of different oligomers, whereas the coiled-coil domain of native laminin-1 is a heterotrimer composed of alpha1, beta1 and gamma1 chains.	bind
41812	2	9890	7	11	NULL	NULL	NULL				folds into			gamma1 deltaN95AE fragments		oligomers	Chemical	mixture of different			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_23_6762_s_205	10581249	A decrease in binding affinity of the recombinant gamma1 chains and the chimeric GCN4 fusion proteins compared with native laminin-1 may be explained in terms of different coiled-coil structures in these molecules: the GCN4 gamma1 chimera folds into homotypic coiled-coil dimers and the gamma1 deltaN95AE fragments into a mixture of different oligomers, whereas the coiled-coil domain of native laminin-1 is a heterotrimer composed of alpha1, beta1 and gamma1 chains.	bind
41813	3	9890	7	11	NULL	NULL	NULL	laminin-1	GP	native	is composed of			coiled-coil domain					alpha1;;beta1;;gamma1		NULL		NULL	NULL	NULL	NULL	gw60_embo_18_23_6762_s_205	10581249	A decrease in binding affinity of the recombinant gamma1 chains and the chimeric GCN4 fusion proteins compared with native laminin-1 may be explained in terms of different coiled-coil structures in these molecules: the GCN4 gamma1 chimera folds into homotypic coiled-coil dimers and the gamma1 deltaN95AE fragments into a mixture of different oligomers, whereas the coiled-coil domain of native laminin-1 is a heterotrimer composed of alpha1, beta1 and gamma1 chains.	bind
34621	1	9891	6	11	NULL	NULL	NULL	cyclin D2 levels	GP	decrease in	results in		might			RB	GP	decreased phosphorylation of 			NULL	WEHI-231 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
34622	2	9891	6	11	NULL	NULL	NULL	cyclin D2 levels	GP	decrease in	results in		might			p107	GP	decreased phosphorylation of			NULL	WEHI-231 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
34623	3	9891	6	11	NULL	NULL	NULL	cyclin D2 levels	GP	decrease in	results in		might			p130	GP	decreased phosphorylation of			NULL	WEHI-231 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
34624	4	9891	6	11	NULL	NULL	NULL	RB	GP		is a type of					pocket protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
34625	5	9891	6	11	NULL	NULL	NULL	p107	GP		is a type of					pocket protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
34626	6	9891	6	11	NULL	NULL	NULL	p130	GP		is a type of					pocket protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
34627	7	9891	6	11	NULL	NULL	NULL	RB	GP		bind					E2F	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
34628	8	9891	6	11	NULL	NULL	NULL	p107	GP		bind					E2F	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
34629	9	9891	6	11	NULL	NULL	NULL	p130	GP		bind					E2F	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
34973	10	9891	6	11	NULL	NULL	NULL	statement 1	Process		results in					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
34974	11	9891	6	11	NULL	NULL	NULL	statement 2	Process		results in					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
34975	12	9891	6	11	NULL	NULL	NULL	statement 3	Process		results in					statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
34976	13	9891	6	11	NULL	NULL	NULL	WEHI-231 cells	Cell		are blocked at					G1-phase restriction point	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
34977	14	9891	6	11	NULL	NULL	NULL	statement 10	Process		leads to					statement 13	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
34978	15	9891	6	11	NULL	NULL	NULL	statement 11	Process		leads to					statement 13	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
34979	16	9891	6	11	NULL	NULL	NULL	statement 12	Process		leads to					statement 13	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
56922	17	9891	6	11	NULL	NULL	NULL	E2F	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
56923	18	9891	6	11	NULL	NULL	NULL	statement 14	Process		inhibits					WEHI-231 cells	Cell	S-phase entry of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
56924	19	9891	6	11	NULL	NULL	NULL	statement 15	Process		inhibits					WEHI-231 cells	Cell	S-phase entry of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
56925	20	9891	6	11	NULL	NULL	NULL	statement 16	Process		inhibits					WEHI-231 cells	Cell	S-phase entry of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
41818	1	9891	7	11	NULL	NULL	NULL	cyclin D2 levels	GP	decrease in	decrease		may			RB	GP	phosphorylation of			NULL	WEHI-231 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
41819	2	9891	7	11	NULL	NULL	NULL	cyclin D2 levels	GP	decrease in	decrease		may			p107	GP	phosphorylation of			NULL	WEHI-231 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
41820	3	9891	7	11	NULL	NULL	NULL	cyclin D2 levels	GP	decrease in	decrease		may			p130	GP	phosphorylation of			NULL	WEHI-231 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
41821	7	9891	7	11	NULL	NULL	NULL	RB	GP		bind					E2F	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
41822	10	9891	7	11	NULL	NULL	NULL	WEHI-231 cells	Cell		are blocked at					G1-phase restriction point	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
41823	11	9891	7	11	NULL	NULL	NULL	statement 16	Process		leads to					statement 10	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
41824	13	9891	7	11	NULL	NULL	NULL	statement 20	Process		inhibits					WEHI-231 cells	Cell	S-phase entry of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
50232	4	9891	7	11	NULL	NULL	NULL	RB	GP		is a type of					pocket protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
50233	5	9891	7	11	NULL	NULL	NULL	p107	GP		is a type of					pocket protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
50234	6	9891	7	11	NULL	NULL	NULL	p130	GP		is a type of					pocket protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
50235	8	9891	7	11	NULL	NULL	NULL	p107	GP		bind					E2F	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
50236	9	9891	7	11	NULL	NULL	NULL	p130	GP		bind					E2F	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
50239	12	9891	7	11	NULL	NULL	NULL	statement 17	Process		leads to					statement 10	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
50240	14	9891	7	11	NULL	NULL	NULL	statement 11	Process		inhibits					WEHI-231 cells	Cell	S-phase entry of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
50241	15	9891	7	11	NULL	NULL	NULL	statement 12	Process		inhibits					WEHI-231 cells	Cell	S-phase entry of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
50243	16	9891	7	11	NULL	NULL	NULL	statement 1	Process		result in					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
50244	17	9891	7	11	NULL	NULL	NULL	statement 2	Process		result in					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
50245	18	9891	7	11	NULL	NULL	NULL	statement 3	Process		result in					statement 9	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
50247	19	9891	7	11	NULL	NULL	NULL	E2F	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
56921	20	9891	7	11	NULL	NULL	NULL	statement 18	Process		leads to					statement 10	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_19_12650_s_253	9139721	A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase ( 93,  95).	bind
34518	1	9892	6	11	NULL	NULL	NULL	Sp100	GP		bind					NB	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_8_2687_s_421	11909962	A decrease in ETS-1 levels would shift the equilibrium toward Sp100 bound to NBs (Fig.  8).	bind
41825	1	9892	7	11	NULL	NULL	NULL	Sp100	GP		bind					NBs	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_8_2687_s_421	11909962	A decrease in ETS-1 levels would shift the equilibrium toward Sp100 bound to NBs (Fig.  8).	bind
34519	1	9893	6	11	NULL	NULL	NULL	PCBP1	GP		bind					66 nt fragment	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_2_639_s_160	12527772	A decrease in mobility of the radiolabelled 292 - 358 fragment was also observed and this would imply that PCBP1 binds to a 66 nt fragment.	bind
41827	1	9893	7	11	NULL	NULL	NULL	PCBP1	GP		binds to					66 nt fragment	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_2_639_s_160	12527772	A decrease in mobility of the radiolabelled 292 - 358 fragment was also observed and this would imply that PCBP1 binds to a 66 nt fragment.	bind
34520	1	9894	6	11	NULL	NULL	NULL	alpha-actinin	GP	phosphorylated	bind					actin filament	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_31_28676_s_342	11369769	A decrease in the binding affinity of phosphorylated alpha-actinin for actin filaments may at least partially explain the disparity between the two alpha-actinin populations.	bind
41828	1	9894	7	11	NULL	NULL	NULL	alpha-actinin	GP	phosphorylated	bind					actin filaments	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_31_28676_s_342	11369769	A decrease in the binding affinity of phosphorylated alpha-actinin for actin filaments may at least partially explain the disparity between the two alpha-actinin populations.	bind
41829	2	9894	7	11	NULL	NULL	NULL	alpha-actinin	GP	disparity between	decrease		may			statement 1	Process	binding affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_31_28676_s_342	11369769	A decrease in the binding affinity of phosphorylated alpha-actinin for actin filaments may at least partially explain the disparity between the two alpha-actinin populations.	bind
34530	1	9895	6	11	NULL	NULL	NULL	villin	GP	phosphorylated	bind					actin filaments	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_39_36163_s_102	11500485	A decrease in the binding affinity of phosphorylated villin for actin filaments may partially explain the redistribution of tyrosine phosphorylated villin  in vivo.	bind
56926	2	9895	6	11	NULL	NULL	NULL	villin	GP	redistribution of;;phosphorylated 	decrease		may	tyrosine		statement 1	Process	binding affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_39_36163_s_102	11500485	A decrease in the binding affinity of phosphorylated villin for actin filaments may partially explain the redistribution of tyrosine phosphorylated villin  in vivo.	bind
41830	1	9895	7	11	NULL	NULL	NULL	villin	GP	phosphorylated	bind					actin filaments	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_39_36163_s_102	11500485	A decrease in the binding affinity of phosphorylated villin for actin filaments may partially explain the redistribution of tyrosine phosphorylated villin  in vivo.	bind
41831	2	9895	7	11	NULL	NULL	NULL	 villin	GP	redistribution of;;phosphorylated 	decrease		may	tyrosine		statement 1	Process	binding affinity of			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_39_36163_s_102	11500485	A decrease in the binding affinity of phosphorylated villin for actin filaments may partially explain the redistribution of tyrosine phosphorylated villin  in vivo.	bind
34533	1	9896	6	11	NULL	NULL	NULL	p52	GP		bind					skp2 gene	GP	proximal		promoter	NULL		NULL	NULL	NULL	NULL	gw70_embo_25_16_3801_s_219	16902410	A decrease in the binding of p52 to the proximal   skp2 gene promoter was observed ( Figure 7F).	bind
41832	1	9896	7	11	NULL	NULL	NULL	 p52	GP		bind					skp2 gene	GP	proximal		promoter	NULL		NULL	NULL	NULL	NULL	gw70_embo_25_16_3801_s_219	16902410	A decrease in the binding of p52 to the proximal   skp2 gene promoter was observed ( Figure 7F).	bind
42295	1	9897	6	11	NULL	NULL	NULL	tc	Chemical		bind					TetR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_11_6936_s_183	9054381	A decrease in the equilibrium binding constant of tc to TetR can be caused by a decrease in the association rate constant, an increase in the dissociation rate constant, or both.	bind
41833	1	9897	7	11	NULL	NULL	NULL	tc	Chemical		bind					TetR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_11_6936_s_183	9054381	A decrease in the equilibrium binding constant of tc to TetR can be caused by a decrease in the association rate constant, an increase in the dissociation rate constant, or both.	bind
34535	1	9898	6	11	NULL	NULL	NULL	CSS	AminoAcid		bind					SCS	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_27_25901_s_212	15888455	A decrease in the GSH/GSSG ratio induced the inhibition of CSS and SCS binding, whereas SSC and SSS binding was not affected ( Fig. 3).	bind
34537	2	9898	6	11	NULL	NULL	NULL	GSH/GSSG ratio	QuantityOrMeasure	decrease in	induces					statement 1	Process	inhibiton of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_27_25901_s_212	15888455	A decrease in the GSH/GSSG ratio induced the inhibition of CSS and SCS binding, whereas SSC and SSS binding was not affected ( Fig. 3).	bind
34538	3	9898	6	11	NULL	NULL	NULL	SSC	AminoAcid		bind					SSS	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_27_25901_s_212	15888455	A decrease in the GSH/GSSG ratio induced the inhibition of CSS and SCS binding, whereas SSC and SSS binding was not affected ( Fig. 3).	bind
34540	4	9898	6	11	NULL	NULL	NULL	GSH/GSSG ratio	QuantityOrMeasure	decrease in	does not affect					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_27_25901_s_212	15888455	A decrease in the GSH/GSSG ratio induced the inhibition of CSS and SCS binding, whereas SSC and SSS binding was not affected ( Fig. 3).	bind
41839	1	9898	7	11	NULL	NULL	NULL	CSS	AminoAcid		bind					SCS	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_27_25901_s_212	15888455	A decrease in the GSH/GSSG ratio induced the inhibition of CSS and SCS binding, whereas SSC and SSS binding was not affected ( Fig. 3).	bind
41840	2	9898	7	11	NULL	NULL	NULL	SSC	AminoAcid		bind					SSS	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_27_25901_s_212	15888455	A decrease in the GSH/GSSG ratio induced the inhibition of CSS and SCS binding, whereas SSC and SSS binding was not affected ( Fig. 3).	bind
41841	3	9898	7	11	NULL	NULL	NULL	GSH/GSSG ratio	QuantityOrMeasure	decrease in	induce					statement 1	Process	inhibition of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_27_25901_s_212	15888455	A decrease in the GSH/GSSG ratio induced the inhibition of CSS and SCS binding, whereas SSC and SSS binding was not affected ( Fig. 3).	bind
41842	4	9898	7	11	NULL	NULL	NULL	GSH/GSSG ratio	QuantityOrMeasure	decrease in	does not affect					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_27_25901_s_212	15888455	A decrease in the GSH/GSSG ratio induced the inhibition of CSS and SCS binding, whereas SSC and SSS binding was not affected ( Fig. 3).	bind
34541	1	9899	6	11	NULL	NULL	NULL	actin	GP		bind					myosin IIA	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_1_121_s_184	16606694	A decrease of actin and myosin IIA binding was seen after treatment with 100 muM of the general protein tyrosine kinase inhibitor genistein (unpublished data), but the observed effects were most likely nonspecific because of the inhibition of all tyrosine kinases and an impairment of NK cell functions.	bind
34542	2	9899	6	11	NULL	NULL	NULL	genistein	Chemical		decreases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_1_121_s_184	16606694	A decrease of actin and myosin IIA binding was seen after treatment with 100 muM of the general protein tyrosine kinase inhibitor genistein (unpublished data), but the observed effects were most likely nonspecific because of the inhibition of all tyrosine kinases and an impairment of NK cell functions.	bind
49004	3	9899	6	11	NULL	NULL	NULL	genistein	Chemical		is a type of					protein tyrosine kinase inhibitor	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_1_121_s_184	16606694	A decrease of actin and myosin IIA binding was seen after treatment with 100 muM of the general protein tyrosine kinase inhibitor genistein (unpublished data), but the observed effects were most likely nonspecific because of the inhibition of all tyrosine kinases and an impairment of NK cell functions.	bind
41843	1	9899	7	11	NULL	NULL	NULL	actin	GP		bind					myosin IIA	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_1_121_s_184	16606694	A decrease of actin and myosin IIA binding was seen after treatment with 100 muM of the general protein tyrosine kinase inhibitor genistein (unpublished data), but the observed effects were most likely nonspecific because of the inhibition of all tyrosine kinases and an impairment of NK cell functions.	bind
41844	2	9899	7	11	NULL	NULL	NULL	genistein	Chemical		decrease					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_1_121_s_184	16606694	A decrease of actin and myosin IIA binding was seen after treatment with 100 muM of the general protein tyrosine kinase inhibitor genistein (unpublished data), but the observed effects were most likely nonspecific because of the inhibition of all tyrosine kinases and an impairment of NK cell functions.	bind
41845	3	9899	7	11	NULL	NULL	NULL	genistein	Chemical		is a type of					protein tyrosine kinase inhibitor	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_1_121_s_184	16606694	A decrease of actin and myosin IIA binding was seen after treatment with 100 muM of the general protein tyrosine kinase inhibitor genistein (unpublished data), but the observed effects were most likely nonspecific because of the inhibition of all tyrosine kinases and an impairment of NK cell functions.	bind
34543	1	9900	6	11	NULL	NULL	NULL	GAPDH	GP		bind					F-actin	GP	skeletal muscle			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_5_821_s_212	8620602	A decrease of ATP concentration has been reported to favor the binding of GAPDH to skeletal muscle F-actin 38  or to tubulin, 39  whereas Mg2+ seems to enhance GAPDH binding to the thin filament from beef muscle.	bind
34544	2	9900	6	11	NULL	NULL	NULL	GAPDH	GP		bind					tubulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_5_821_s_212	8620602	A decrease of ATP concentration has been reported to favor the binding of GAPDH to skeletal muscle F-actin 38  or to tubulin, 39  whereas Mg2+ seems to enhance GAPDH binding to the thin filament from beef muscle.	bind
34545	3	9900	6	11	NULL	NULL	NULL	ATP concentration	Chemical	decrease of	favors					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_5_821_s_212	8620602	A decrease of ATP concentration has been reported to favor the binding of GAPDH to skeletal muscle F-actin 38  or to tubulin, 39  whereas Mg2+ seems to enhance GAPDH binding to the thin filament from beef muscle.	bind
34546	4	9900	6	11	NULL	NULL	NULL	ATP concentration	Chemical	decrease of	favors					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_5_821_s_212	8620602	A decrease of ATP concentration has been reported to favor the binding of GAPDH to skeletal muscle F-actin 38  or to tubulin, 39  whereas Mg2+ seems to enhance GAPDH binding to the thin filament from beef muscle.	bind
34547	5	9900	6	11	NULL	NULL	NULL	GAPDH	GP		bind					thin filament	GP	beef			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_5_821_s_212	8620602	A decrease of ATP concentration has been reported to favor the binding of GAPDH to skeletal muscle F-actin 38  or to tubulin, 39  whereas Mg2+ seems to enhance GAPDH binding to the thin filament from beef muscle.	bind
34548	6	9900	6	11	NULL	NULL	NULL	Mg2+	Chemical		enhances					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_5_821_s_212	8620602	A decrease of ATP concentration has been reported to favor the binding of GAPDH to skeletal muscle F-actin 38  or to tubulin, 39  whereas Mg2+ seems to enhance GAPDH binding to the thin filament from beef muscle.	bind
41848	1	9900	7	11	NULL	NULL	NULL	GAPDH	GP		bind					F-actin	GP	skeletal muscle			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_5_821_s_212	8620602	A decrease of ATP concentration has been reported to favor the binding of GAPDH to skeletal muscle F-actin 38  or to tubulin, 39  whereas Mg2+ seems to enhance GAPDH binding to the thin filament from beef muscle.	bind
41849	2	9900	7	11	NULL	NULL	NULL	GAPDH	GP		bind					tubulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_5_821_s_212	8620602	A decrease of ATP concentration has been reported to favor the binding of GAPDH to skeletal muscle F-actin 38  or to tubulin, 39  whereas Mg2+ seems to enhance GAPDH binding to the thin filament from beef muscle.	bind
41850	3	9900	7	11	NULL	NULL	NULL	ATP	Chemical	decrease in	favors					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_5_821_s_212	8620602	A decrease of ATP concentration has been reported to favor the binding of GAPDH to skeletal muscle F-actin 38  or to tubulin, 39  whereas Mg2+ seems to enhance GAPDH binding to the thin filament from beef muscle.	bind
41851	4	9900	7	11	NULL	NULL	NULL	ATP	Chemical	decrease in	favors					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_5_821_s_212	8620602	A decrease of ATP concentration has been reported to favor the binding of GAPDH to skeletal muscle F-actin 38  or to tubulin, 39  whereas Mg2+ seems to enhance GAPDH binding to the thin filament from beef muscle.	bind
41852	5	9900	7	11	NULL	NULL	NULL	GAPDH	GP		bind					thin filament	GP	beef muscle			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_5_821_s_212	8620602	A decrease of ATP concentration has been reported to favor the binding of GAPDH to skeletal muscle F-actin 38  or to tubulin, 39  whereas Mg2+ seems to enhance GAPDH binding to the thin filament from beef muscle.	bind
41853	6	9900	7	11	NULL	NULL	NULL	Mg2+	Chemical		enhance					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_78_5_821_s_212	8620602	A decrease of ATP concentration has been reported to favor the binding of GAPDH to skeletal muscle F-actin 38  or to tubulin, 39  whereas Mg2+ seems to enhance GAPDH binding to the thin filament from beef muscle.	bind
34549	1	9901	6	11	NULL	NULL	NULL	SRF + SAP-1 complex	GP		bind					c-fos	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_98_1_78_s_50	8690807	A decreased binding of the SRF + SAP-1 complex to the  c-fos promotor, would probably lead to  a decreased transcription of the  c-fos gene, followed by a subsequent decrease of the DNA-binding of AP-1 to the  c-fos  promotor.	bind
34550	2	9901	6	11	NULL	NULL	NULL	statement 1	Process	decrease in	decreases					c-fos gene	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_98_1_78_s_50	8690807	A decreased binding of the SRF + SAP-1 complex to the  c-fos promotor, would probably lead to  a decreased transcription of the  c-fos gene, followed by a subsequent decrease of the DNA-binding of AP-1 to the  c-fos  promotor.	bind
34551	3	9901	6	11	NULL	NULL	NULL	AP-1	GP		bind					c-fos	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_98_1_78_s_50	8690807	A decreased binding of the SRF + SAP-1 complex to the  c-fos promotor, would probably lead to  a decreased transcription of the  c-fos gene, followed by a subsequent decrease of the DNA-binding of AP-1 to the  c-fos  promotor.	bind
34552	4	9901	6	11	NULL	NULL	NULL	statement 2	Process		leads to					statement 3	Process	decrease in			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_98_1_78_s_50	8690807	A decreased binding of the SRF + SAP-1 complex to the  c-fos promotor, would probably lead to  a decreased transcription of the  c-fos gene, followed by a subsequent decrease of the DNA-binding of AP-1 to the  c-fos  promotor.	bind
41854	1	9901	7	11	NULL	NULL	NULL	SRF + SAP-1 complex	GP		bind					c-fos	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_98_1_78_s_50	8690807	A decreased binding of the SRF + SAP-1 complex to the  c-fos promotor, would probably lead to  a decreased transcription of the  c-fos gene, followed by a subsequent decrease of the DNA-binding of AP-1 to the  c-fos  promotor.	bind
41855	2	9901	7	11	NULL	NULL	NULL	statement 1	Process		lead to					c-fos gene	GP	 transcription of 			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_98_1_78_s_50	8690807	A decreased binding of the SRF + SAP-1 complex to the  c-fos promotor, would probably lead to  a decreased transcription of the  c-fos gene, followed by a subsequent decrease of the DNA-binding of AP-1 to the  c-fos  promotor.	bind
41857	3	9901	7	11	NULL	NULL	NULL	AP-1	GP		bind					c-fos	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_98_1_78_s_50	8690807	A decreased binding of the SRF + SAP-1 complex to the  c-fos promotor, would probably lead to  a decreased transcription of the  c-fos gene, followed by a subsequent decrease of the DNA-binding of AP-1 to the  c-fos  promotor.	bind
41861	4	9901	7	11	NULL	NULL	NULL	statement 1	Process	decrease of	lead to					statement 2	Process	decrease of			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_98_1_78_s_50	8690807	A decreased binding of the SRF + SAP-1 complex to the  c-fos promotor, would probably lead to  a decreased transcription of the  c-fos gene, followed by a subsequent decrease of the DNA-binding of AP-1 to the  c-fos  promotor.	bind
41862	5	9901	7	11	NULL	NULL	NULL	statement 2	Process	decrease of	lead to					statement 3	Process	decrease of			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_98_1_78_s_50	8690807	A decreased binding of the SRF + SAP-1 complex to the  c-fos promotor, would probably lead to  a decreased transcription of the  c-fos gene, followed by a subsequent decrease of the DNA-binding of AP-1 to the  c-fos  promotor.	bind
34980	1	9902	6	11	NULL	NULL	NULL			positively charged	bind		likely	pocket S2					aspartic acid located N terminal to the cleavage site		NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_1_302_s_10	14694194	A deep and positively charged pocket (S2) and a neighboring shallow surface (S3) likely bind to aspartic acid and glycine residues in the substrate located two (P2) and three (P3) residues N terminal to the cleavage site, respectively.	bind
34981	2	9902	6	11	NULL	NULL	NULL			positively charged	bind		likely	pocket S2					glycine residues N terminal to the cleavage site		NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_1_302_s_10	14694194	A deep and positively charged pocket (S2) and a neighboring shallow surface (S3) likely bind to aspartic acid and glycine residues in the substrate located two (P2) and three (P3) residues N terminal to the cleavage site, respectively.	bind
34982	3	9902	6	11	NULL	NULL	NULL				bind		likely	shallow surface S3					aspartic acid located N terminal to the cleavage site		NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_1_302_s_10	14694194	A deep and positively charged pocket (S2) and a neighboring shallow surface (S3) likely bind to aspartic acid and glycine residues in the substrate located two (P2) and three (P3) residues N terminal to the cleavage site, respectively.	bind
34983	4	9902	6	11	NULL	NULL	NULL				bind		likely	shallow surface S3					glycine residues N terminal to the cleavage site		NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_1_302_s_10	14694194	A deep and positively charged pocket (S2) and a neighboring shallow surface (S3) likely bind to aspartic acid and glycine residues in the substrate located two (P2) and three (P3) residues N terminal to the cleavage site, respectively.	bind
41863	1	9902	7	11	NULL	NULL	NULL			positively charged	bind			S2 pocket					aspartic acid located N terminal to the cleavage site		NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_1_302_s_10	14694194	A deep and positively charged pocket (S2) and a neighboring shallow surface (S3) likely bind to aspartic acid and glycine residues in the substrate located two (P2) and three (P3) residues N terminal to the cleavage site, respectively.	bind
41864	2	9902	7	11	NULL	NULL	NULL			positively charged	bind			S2 pocket					glycine located N terminal to the cleavage site		NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_1_302_s_10	14694194	A deep and positively charged pocket (S2) and a neighboring shallow surface (S3) likely bind to aspartic acid and glycine residues in the substrate located two (P2) and three (P3) residues N terminal to the cleavage site, respectively.	bind
41865	3	9902	7	11	NULL	NULL	NULL				bind			shallow surface S3					aspartic acid located N terminal to the cleavage site		NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_1_302_s_10	14694194	A deep and positively charged pocket (S2) and a neighboring shallow surface (S3) likely bind to aspartic acid and glycine residues in the substrate located two (P2) and three (P3) residues N terminal to the cleavage site, respectively.	bind
41866	4	9902	7	11	NULL	NULL	NULL				bind			shallow surface S3					glycine located N terminal to the cleavage site		NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_1_302_s_10	14694194	A deep and positively charged pocket (S2) and a neighboring shallow surface (S3) likely bind to aspartic acid and glycine residues in the substrate located two (P2) and three (P3) residues N terminal to the cleavage site, respectively.	bind
34553	1	9904	6	11	NULL	NULL	NULL	CPF	GP		bind							unphosphorylated	CTD		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_8_1030_s_334	12704082	A defect in binding of CPF to unphosphorylated CTD may trigger a very specific removal of Pta1.	bind
34554	2	9904	6	11	NULL	NULL	NULL	statement 1	Process	defect in	trigger		may			Pta1	GP	removal of			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_8_1030_s_334	12704082	A defect in binding of CPF to unphosphorylated CTD may trigger a very specific removal of Pta1.	bind
41873	1	9904	7	11	NULL	NULL	NULL	CPF	GP		bind							unphosphorylated 	CTD		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_8_1030_s_334	12704082	A defect in binding of CPF to unphosphorylated CTD may trigger a very specific removal of Pta1.	bind
41874	2	9904	7	11	NULL	NULL	NULL	statement 1	Process	defect in	trigger					Pta1	GP	removal of			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_8_1030_s_334	12704082	A defect in binding of CPF to unphosphorylated CTD may trigger a very specific removal of Pta1.	bind
34618	1	9905	6	11	NULL	NULL	NULL	mucin	GP	deficiency in production of	compromise		may			intestinal barrier	OrganismPart	function of			NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_24_3_353_s_29	12663492	A deficiency in mucin production, or altered mucin structure and lectin binding, could also compromise intestinal barrier function ( , ).	bind
34619	2	9905	6	11	NULL	NULL	NULL	mucin	GP	altered;;structure of	compromise		may			intestinal barrier	OrganismPart	function of			NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_24_3_353_s_29	12663492	A deficiency in mucin production, or altered mucin structure and lectin binding, could also compromise intestinal barrier function ( , ).	bind
34620	3	9905	6	11	NULL	NULL	NULL	lectin	GP	binding of	compromise		may			intestinal barrier	OrganismPart	function of			NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_24_3_353_s_29	12663492	A deficiency in mucin production, or altered mucin structure and lectin binding, could also compromise intestinal barrier function ( , ).	bind
41905	1	9905	7	11	NULL	NULL	NULL	mucin	GP	deficiency in production of	compromise		may			intestinal barrier	OrganismPart	function of			NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_24_3_353_s_29	12663492	A deficiency in mucin production, or altered mucin structure and lectin binding, could also compromise intestinal barrier function ( , ).	bind
41906	2	9905	7	11	NULL	NULL	NULL	mucin	GP	altered;;structure of	compromise		may			intestinal barrier	OrganismPart	function of			NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_24_3_353_s_29	12663492	A deficiency in mucin production, or altered mucin structure and lectin binding, could also compromise intestinal barrier function ( , ).	bind
41907	3	9905	7	11	NULL	NULL	NULL	lectin	GP	binding of	compromise		may			intestinal barrier	OrganismPart	function of			NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_24_3_353_s_29	12663492	A deficiency in mucin production, or altered mucin structure and lectin binding, could also compromise intestinal barrier function ( , ).	bind
34555	1	9906	6	11	NULL	NULL	NULL	GAG chain	NucleicAcid		bind			pentasaccharide sequence		antithrombin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_25_15487_s_13	9624135	A defined pentasaccharide sequence in the GAG chain binds antithrombin and thus strongly promotes its function as an inhibitor of the serine proteases acting within the coagulation cascade ( 2).	bind
34556	2	9906	6	11	NULL	NULL	NULL	antithrombin	GP		functions as					serine proteases	GP	inhibitor of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_25_15487_s_13	9624135	A defined pentasaccharide sequence in the GAG chain binds antithrombin and thus strongly promotes its function as an inhibitor of the serine proteases acting within the coagulation cascade ( 2).	bind
34557	3	9906	6	11	NULL	NULL	NULL	statement 2	Process		occurs within					coagulation cascade	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_25_15487_s_13	9624135	A defined pentasaccharide sequence in the GAG chain binds antithrombin and thus strongly promotes its function as an inhibitor of the serine proteases acting within the coagulation cascade ( 2).	bind
34558	4	9906	6	11	NULL	NULL	NULL	statement 1	Process		promotes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_25_15487_s_13	9624135	A defined pentasaccharide sequence in the GAG chain binds antithrombin and thus strongly promotes its function as an inhibitor of the serine proteases acting within the coagulation cascade ( 2).	bind
41875	1	9906	7	11	NULL	NULL	NULL	GAG chain	NucleicAcid		binds			pentasaccharide sequence 		antithrombin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_25_15487_s_13	9624135	A defined pentasaccharide sequence in the GAG chain binds antithrombin and thus strongly promotes its function as an inhibitor of the serine proteases acting within the coagulation cascade ( 2).	bind
41876	2	9906	7	11	NULL	NULL	NULL	statement 1	Process		promotes					antithrombin	GP	function of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_25_15487_s_13	9624135	A defined pentasaccharide sequence in the GAG chain binds antithrombin and thus strongly promotes its function as an inhibitor of the serine proteases acting within the coagulation cascade ( 2).	bind
41877	3	9906	7	11	NULL	NULL	NULL	antithrombin	GP		functions as					serine proteases	GP	inhibitor of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_25_15487_s_13	9624135	A defined pentasaccharide sequence in the GAG chain binds antithrombin and thus strongly promotes its function as an inhibitor of the serine proteases acting within the coagulation cascade ( 2).	bind
41878	4	9906	7	11	NULL	NULL	NULL	statement 3	Process		occurs within					coagulation cascade	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_25_15487_s_13	9624135	A defined pentasaccharide sequence in the GAG chain binds antithrombin and thus strongly promotes its function as an inhibitor of the serine proteases acting within the coagulation cascade ( 2).	bind
34559	1	9907	6	11	NULL	NULL	NULL	Ran GTPase	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_24_3011_s_112	14681208	A defining characteristic of karyopherins that function in nuclear export is that cargo binding requires the GTP-bound form of the Ran GTPase (Lei and Silver 2002 ).	bind
34560	2	9907	6	11	NULL	NULL	NULL	karyopherins	GP		function in					nuclear export	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_24_3011_s_112	14681208	A defining characteristic of karyopherins that function in nuclear export is that cargo binding requires the GTP-bound form of the Ran GTPase (Lei and Silver 2002 ).	bind
34561	3	9907	6	11	NULL	NULL	NULL	cargo	GP	binding of	requires					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_24_3011_s_112	14681208	A defining characteristic of karyopherins that function in nuclear export is that cargo binding requires the GTP-bound form of the Ran GTPase (Lei and Silver 2002 ).	bind
41879	1	9907	7	11	NULL	NULL	NULL	karyopherins	GP		function in					nuclear export	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_24_3011_s_112	14681208	A defining characteristic of karyopherins that function in nuclear export is that cargo binding requires the GTP-bound form of the Ran GTPase (Lei and Silver 2002 ).	bind
41880	3	9907	7	11	NULL	NULL	NULL	cargo	GP	binding of	requires					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_24_3011_s_112	14681208	A defining characteristic of karyopherins that function in nuclear export is that cargo binding requires the GTP-bound form of the Ran GTPase (Lei and Silver 2002 ).	bind
41881	2	9907	7	11	NULL	NULL	NULL	GTP	Chemical		bind					Ran GTPase	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_24_3011_s_112	14681208	A defining characteristic of karyopherins that function in nuclear export is that cargo binding requires the GTP-bound form of the Ran GTPase (Lei and Silver 2002 ).	bind
34562	1	9908	6	11	NULL	NULL	NULL	karyopherins	GP		function in					nuclear export	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_24_3011_s_29	14681208	A defining characteristic of karyopherins that function in nuclear export is that nuclear cargo binding requires the GTP-bound form of the Ran GTPase, whereas cytoplasmic hydrolysis of Ran-GTP to Ran-GDP induces cargo release.	bind
34563	2	9908	6	11	NULL	NULL	NULL	GTP	Chemical		bind					Ran GTPase	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_24_3011_s_29	14681208	A defining characteristic of karyopherins that function in nuclear export is that nuclear cargo binding requires the GTP-bound form of the Ran GTPase, whereas cytoplasmic hydrolysis of Ran-GTP to Ran-GDP induces cargo release.	bind
34564	3	9908	6	11	NULL	NULL	NULL	cargo	GP	binding of;;nuclear	requires					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_24_3011_s_29	14681208	A defining characteristic of karyopherins that function in nuclear export is that nuclear cargo binding requires the GTP-bound form of the Ran GTPase, whereas cytoplasmic hydrolysis of Ran-GTP to Ran-GDP induces cargo release.	bind
34565	4	9908	6	11	NULL	NULL	NULL	Ran-GTP	Chemical		is hydrolysed to					Ran-GDP	Chemical				NULL	cytoplasm	NULL	NULL	NULL	NULL	gw70_genesdev_17_24_3011_s_29	14681208	A defining characteristic of karyopherins that function in nuclear export is that nuclear cargo binding requires the GTP-bound form of the Ran GTPase, whereas cytoplasmic hydrolysis of Ran-GTP to Ran-GDP induces cargo release.	bind
34566	5	9908	6	11	NULL	NULL	NULL	statement 4	Process		induces					cargo release	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_24_3011_s_29	14681208	A defining characteristic of karyopherins that function in nuclear export is that nuclear cargo binding requires the GTP-bound form of the Ran GTPase, whereas cytoplasmic hydrolysis of Ran-GTP to Ran-GDP induces cargo release.	bind
41882	1	9908	7	11	NULL	NULL	NULL	karyopherins 	GP		function in					nuclear export	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_24_3011_s_29	14681208	A defining characteristic of karyopherins that function in nuclear export is that nuclear cargo binding requires the GTP-bound form of the Ran GTPase, whereas cytoplasmic hydrolysis of Ran-GTP to Ran-GDP induces cargo release.	bind
41883	2	9908	7	11	NULL	NULL	NULL	GTP	Chemical		bind					Ran GTPase	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_24_3011_s_29	14681208	A defining characteristic of karyopherins that function in nuclear export is that nuclear cargo binding requires the GTP-bound form of the Ran GTPase, whereas cytoplasmic hydrolysis of Ran-GTP to Ran-GDP induces cargo release.	bind
41884	3	9908	7	11	NULL	NULL	NULL	cargo	GP	binding of;;nuclear	requires					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_24_3011_s_29	14681208	A defining characteristic of karyopherins that function in nuclear export is that nuclear cargo binding requires the GTP-bound form of the Ran GTPase, whereas cytoplasmic hydrolysis of Ran-GTP to Ran-GDP induces cargo release.	bind
41885	4	9908	7	11	NULL	NULL	NULL	Ran-GTP	Chemical		hydrolyse to					Ran-GDP	Chemical				NULL	cytoplasm	NULL	NULL	NULL	NULL	gw70_genesdev_17_24_3011_s_29	14681208	A defining characteristic of karyopherins that function in nuclear export is that nuclear cargo binding requires the GTP-bound form of the Ran GTPase, whereas cytoplasmic hydrolysis of Ran-GTP to Ran-GDP induces cargo release.	bind
41886	5	9908	7	11	NULL	NULL	NULL	statement 4	Process		induce					cargo release	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_24_3011_s_29	14681208	A defining characteristic of karyopherins that function in nuclear export is that nuclear cargo binding requires the GTP-bound form of the Ran GTPase, whereas cytoplasmic hydrolysis of Ran-GTP to Ran-GDP induces cargo release.	bind
34567	1	9909	6	11	NULL	NULL	NULL	mAspAT	GP	refolding	bind					groEL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_3_1138_s_402	7836372	A definitive answer to the question of why refolding mAspAT binds  more tightly to groEL than its homologous isozymic counterpart awaits  an analysis of the structure of the complex between groEL and its  passenger protein.	bind
34569	3	9909	6	11	NULL	NULL	NULL	statement 1	Process	affinity of	is higher than					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_3_1138_s_402	7836372	A definitive answer to the question of why refolding mAspAT binds  more tightly to groEL than its homologous isozymic counterpart awaits  an analysis of the structure of the complex between groEL and its  passenger protein.	bind
49534	2	9909	6	11	NULL	NULL	NULL	mAspAT	GP		bind					GroEL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_3_1138_s_402	7836372	A definitive answer to the question of why refolding mAspAT binds  more tightly to groEL than its homologous isozymic counterpart awaits  an analysis of the structure of the complex between groEL and its  passenger protein.	bind
41887	1	9909	7	11	NULL	NULL	NULL	mAspAT	GP	refolding	bind		tightly			groEL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_3_1138_s_402	7836372	A definitive answer to the question of why refolding mAspAT binds  more tightly to groEL than its homologous isozymic counterpart awaits  an analysis of the structure of the complex between groEL and its  passenger protein.	bind
49550	2	9909	7	11	NULL	NULL	NULL	 mAspAT	GP		bind					groEL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_3_1138_s_402	7836372	A definitive answer to the question of why refolding mAspAT binds  more tightly to groEL than its homologous isozymic counterpart awaits  an analysis of the structure of the complex between groEL and its  passenger protein.	bind
49551	3	9909	7	11	NULL	NULL	NULL	statement 1	Process	affinity of	is higher than					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_3_1138_s_402	7836372	A definitive answer to the question of why refolding mAspAT binds  more tightly to groEL than its homologous isozymic counterpart awaits  an analysis of the structure of the complex between groEL and its  passenger protein.	bind
42296	1	9910	6	11	NULL	NULL	NULL	ERK2	GP		undergoes			Tyr185		phosphorylation	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_40817_s_215	11524422	A definitive correlation between Tyr185 phosphorylation, changes in enzyme structure, and ATP binding must necessarily await a crystal structure of [Tyr(P)185]ERK2.	bind
42299	1	9910	7	11	NULL	NULL	NULL	ERK2	GP		undergoes			Tyr185		phosphorylation	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_40817_s_215	11524422	A definitive correlation between Tyr185 phosphorylation, changes in enzyme structure, and ATP binding must necessarily await a crystal structure of [Tyr(P)185]ERK2.	bind
34570	1	9912	6	11	NULL	NULL	NULL	COP1	GP		bind			coiled coil domain		SPA1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_41_38173_s_129	11461903	A deletion derivative of COP1 lacking the coiled-coil domain (COP1-deltacc) did not exhibit any detectable interaction with SPA1, indicating that the coiled-coil domain of COP1 is necessary for the SPA1 binding activity of COP1.	bind
34572	2	9912	6	11	NULL	NULL	NULL	COP1-deltacc	GP		is					deletion derivative of COP1 lacking the coiled-coil domain	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_41_38173_s_129	11461903	A deletion derivative of COP1 lacking the coiled-coil domain (COP1-deltacc) did not exhibit any detectable interaction with SPA1, indicating that the coiled-coil domain of COP1 is necessary for the SPA1 binding activity of COP1.	bind
34573	3	9912	6	11	NULL	NULL	NULL	COP1-deltacc	GP		does not interact with					SPA1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_41_38173_s_129	11461903	A deletion derivative of COP1 lacking the coiled-coil domain (COP1-deltacc) did not exhibit any detectable interaction with SPA1, indicating that the coiled-coil domain of COP1 is necessary for the SPA1 binding activity of COP1.	bind
41890	1	9912	7	11	NULL	NULL	NULL	COP1-deltacc	GP		does not interact with					SPA1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_41_38173_s_129	11461903	A deletion derivative of COP1 lacking the coiled-coil domain (COP1-deltacc) did not exhibit any detectable interaction with SPA1, indicating that the coiled-coil domain of COP1 is necessary for the SPA1 binding activity of COP1.	bind
41891	2	9912	7	11	NULL	NULL	NULL	COP1-deltacc	GP		is					deletion derivative lacking coiled-coil domain COP1 	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_41_38173_s_129	11461903	A deletion derivative of COP1 lacking the coiled-coil domain (COP1-deltacc) did not exhibit any detectable interaction with SPA1, indicating that the coiled-coil domain of COP1 is necessary for the SPA1 binding activity of COP1.	bind
41892	3	9912	7	11	NULL	NULL	NULL	COP1	GP		bind			coiled-coil domain		SPA1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_41_38173_s_129	11461903	A deletion derivative of COP1 lacking the coiled-coil domain (COP1-deltacc) did not exhibit any detectable interaction with SPA1, indicating that the coiled-coil domain of COP1 is necessary for the SPA1 binding activity of COP1.	bind
34615	1	9913	6	11	NULL	NULL	NULL	PDGF	GP		is					platelet-derived growth factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2395_s_328	9409207	A deletion in the extracellular domain of the alpha platelet-derived growth factor (PDGF) receptor differentially impairs PDGF-AA and PDGF-BB binding affinities.	bind
34616	2	9913	6	11	NULL	NULL	NULL	PDGF alpha receptor	GP	deletion of	impairs		differentially	extracellular domain		PDGF-AA	GP	binding affinity of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2395_s_328	9409207	A deletion in the extracellular domain of the alpha platelet-derived growth factor (PDGF) receptor differentially impairs PDGF-AA and PDGF-BB binding affinities.	bind
34617	3	9913	6	11	NULL	NULL	NULL	PDGF alpha receptor	GP	deletion of	impairs		differentially	extracellular domain		PDGF-BB	GP	binding affinity of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2395_s_328	9409207	A deletion in the extracellular domain of the alpha platelet-derived growth factor (PDGF) receptor differentially impairs PDGF-AA and PDGF-BB binding affinities.	bind
41893	1	9913	7	11	NULL	NULL	NULL	alpha PDGF receptor	GP	deletion in	impairs		differentially	 extracellular domain 		PDGF-AA	GP	binding affinity of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2395_s_328	9409207	A deletion in the extracellular domain of the alpha platelet-derived growth factor (PDGF) receptor differentially impairs PDGF-AA and PDGF-BB binding affinities.	bind
41894	2	9913	7	11	NULL	NULL	NULL	alpha PDGF receptor	GP	deletion in	impairs		differentially	extracellular domain		PDGF-BB	GP	binding affinity of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2395_s_328	9409207	A deletion in the extracellular domain of the alpha platelet-derived growth factor (PDGF) receptor differentially impairs PDGF-AA and PDGF-BB binding affinities.	bind
41895	3	9913	7	11	NULL	NULL	NULL	PDGF	GP		is					platelet-derived growth factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_11_2395_s_328	9409207	A deletion in the extracellular domain of the alpha platelet-derived growth factor (PDGF) receptor differentially impairs PDGF-AA and PDGF-BB binding affinities.	bind
34611	1	9914	6	11	NULL	NULL	NULL	Scd1	GP		bind					Klp5/6	GP				NULL		NULL	NULL	NULL	NULL	gw70_genetics_165_2_477_s_8	14573463	A deletion in the Scd1 C terminus, which contains the PB1 domain, prevented Scd1 binding to Klp5/6 and caused a growth defect in Klp5/6 mutant cells that is indistinguishable from that induced by  scd1delta.	bind
34612	2	9914	6	11	NULL	NULL	NULL	Scd1	GP		contains			C terminus					PB1 domain		NULL		NULL	NULL	NULL	NULL	gw70_genetics_165_2_477_s_8	14573463	A deletion in the Scd1 C terminus, which contains the PB1 domain, prevented Scd1 binding to Klp5/6 and caused a growth defect in Klp5/6 mutant cells that is indistinguishable from that induced by  scd1delta.	bind
34613	3	9914	6	11	NULL	NULL	NULL	Scd1	GP	deletion of	prevents			C terminus		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_genetics_165_2_477_s_8	14573463	A deletion in the Scd1 C terminus, which contains the PB1 domain, prevented Scd1 binding to Klp5/6 and caused a growth defect in Klp5/6 mutant cells that is indistinguishable from that induced by  scd1delta.	bind
34614	4	9914	6	11	NULL	NULL	NULL	Scd1	GP	deletion of	causes			C terminus		Klp5/6 mutant cells	Cell	growth defect in			NULL		NULL	NULL	NULL	NULL	gw70_genetics_165_2_477_s_8	14573463	A deletion in the Scd1 C terminus, which contains the PB1 domain, prevented Scd1 binding to Klp5/6 and caused a growth defect in Klp5/6 mutant cells that is indistinguishable from that induced by  scd1delta.	bind
49005	5	9914	6	11	NULL	NULL	NULL	scd1delta	GP		induces					growth defect	Process				NULL	Klp5/6 mutant cells	NULL	NULL	NULL	NULL	gw70_genetics_165_2_477_s_8	14573463	A deletion in the Scd1 C terminus, which contains the PB1 domain, prevented Scd1 binding to Klp5/6 and caused a growth defect in Klp5/6 mutant cells that is indistinguishable from that induced by  scd1delta.	bind
41896	1	9914	7	11	NULL	NULL	NULL	Scd1	GP		bind					Klp5/6	Cell				NULL		NULL	NULL	NULL	NULL	gw70_genetics_165_2_477_s_8	14573463	A deletion in the Scd1 C terminus, which contains the PB1 domain, prevented Scd1 binding to Klp5/6 and caused a growth defect in Klp5/6 mutant cells that is indistinguishable from that induced by  scd1delta.	bind
41897	2	9914	7	11	NULL	NULL	NULL	 Scd1	GP		contains			C terminus					PB1 domain		NULL		NULL	NULL	NULL	NULL	gw70_genetics_165_2_477_s_8	14573463	A deletion in the Scd1 C terminus, which contains the PB1 domain, prevented Scd1 binding to Klp5/6 and caused a growth defect in Klp5/6 mutant cells that is indistinguishable from that induced by  scd1delta.	bind
41898	3	9914	7	11	NULL	NULL	NULL	Scd1	GP	deletion of	prevents 			C terminus		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_genetics_165_2_477_s_8	14573463	A deletion in the Scd1 C terminus, which contains the PB1 domain, prevented Scd1 binding to Klp5/6 and caused a growth defect in Klp5/6 mutant cells that is indistinguishable from that induced by  scd1delta.	bind
41899	4	9914	7	11	NULL	NULL	NULL	statement 3	Process		cause					Klp5/6 mutant cells	Cell	growth defect in			NULL		NULL	NULL	NULL	NULL	gw70_genetics_165_2_477_s_8	14573463	A deletion in the Scd1 C terminus, which contains the PB1 domain, prevented Scd1 binding to Klp5/6 and caused a growth defect in Klp5/6 mutant cells that is indistinguishable from that induced by  scd1delta.	bind
41900	5	9914	7	11	NULL	NULL	NULL	scd1delta	GP		induce					growth defect	Process				NULL	Klp5/6 mutant cells	NULL	NULL	NULL	NULL	gw70_genetics_165_2_477_s_8	14573463	A deletion in the Scd1 C terminus, which contains the PB1 domain, prevented Scd1 binding to Klp5/6 and caused a growth defect in Klp5/6 mutant cells that is indistinguishable from that induced by  scd1delta.	bind
34609	1	9915	6	11	NULL	NULL	NULL	G protein	GP		bind					FPR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_39_27934_s_152	10488141	A deletion including three threonine and one serine residue, delta330-336, caused a significant decrease in G protein coupling, supporting previously obtained results showing that a synthetic peptide corresponding to amino acids 322-336 inhibits binding of G protein to FPR (Fig.  1 A) ( 5,  6).	bind
34610	2	9915	6	11	NULL	NULL	NULL	synthetic peptide	Chemical		inhibits			amino acids 322-336		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_39_27934_s_152	10488141	A deletion including three threonine and one serine residue, delta330-336, caused a significant decrease in G protein coupling, supporting previously obtained results showing that a synthetic peptide corresponding to amino acids 322-336 inhibits binding of G protein to FPR (Fig.  1 A) ( 5,  6).	bind
49007	3	9915	6	11	NULL	NULL	NULL	delta330-336	AminoAcid		includes					threonine and serine residue	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_39_27934_s_152	10488141	A deletion including three threonine and one serine residue, delta330-336, caused a significant decrease in G protein coupling, supporting previously obtained results showing that a synthetic peptide corresponding to amino acids 322-336 inhibits binding of G protein to FPR (Fig.  1 A) ( 5,  6).	bind
49008	4	9915	6	11	NULL	NULL	NULL	statement 3	Process		decreases					G protein coupling	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_39_27934_s_152	10488141	A deletion including three threonine and one serine residue, delta330-336, caused a significant decrease in G protein coupling, supporting previously obtained results showing that a synthetic peptide corresponding to amino acids 322-336 inhibits binding of G protein to FPR (Fig.  1 A) ( 5,  6).	bind
49009	5	9915	6	11	NULL	NULL	NULL	statement 4	Process		supports					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_39_27934_s_152	10488141	A deletion including three threonine and one serine residue, delta330-336, caused a significant decrease in G protein coupling, supporting previously obtained results showing that a synthetic peptide corresponding to amino acids 322-336 inhibits binding of G protein to FPR (Fig.  1 A) ( 5,  6).	bind
41901	1	9915	7	11	NULL	NULL	NULL	G protein	GP		bind					FPR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_39_27934_s_152	10488141	A deletion including three threonine and one serine residue, delta330-336, caused a significant decrease in G protein coupling, supporting previously obtained results showing that a synthetic peptide corresponding to amino acids 322-336 inhibits binding of G protein to FPR (Fig.  1 A) ( 5,  6).	bind
41902	2	9915	7	11	NULL	NULL	NULL	synthetic peptide	Chemical		inhibits			amino acids 322-336		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_39_27934_s_152	10488141	A deletion including three threonine and one serine residue, delta330-336, caused a significant decrease in G protein coupling, supporting previously obtained results showing that a synthetic peptide corresponding to amino acids 322-336 inhibits binding of G protein to FPR (Fig.  1 A) ( 5,  6).	bind
41903	4	9915	7	11	NULL	NULL	NULL	statement 3	Process		decrease					G protein coupling	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_39_27934_s_152	10488141	A deletion including three threonine and one serine residue, delta330-336, caused a significant decrease in G protein coupling, supporting previously obtained results showing that a synthetic peptide corresponding to amino acids 322-336 inhibits binding of G protein to FPR (Fig.  1 A) ( 5,  6).	bind
41904	5	9915	7	11	NULL	NULL	NULL	statement 4	Process		support					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_39_27934_s_152	10488141	A deletion including three threonine and one serine residue, delta330-336, caused a significant decrease in G protein coupling, supporting previously obtained results showing that a synthetic peptide corresponding to amino acids 322-336 inhibits binding of G protein to FPR (Fig.  1 A) ( 5,  6).	bind
49006	3	9915	7	11	NULL	NULL	NULL	delta330-336	AminoAcid		includes					threonine and serine residue	AminoAcid	deletion of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_39_27934_s_152	10488141	A deletion including three threonine and one serine residue, delta330-336, caused a significant decrease in G protein coupling, supporting previously obtained results showing that a synthetic peptide corresponding to amino acids 322-336 inhibits binding of G protein to FPR (Fig.  1 A) ( 5,  6).	bind
34605	1	9916	6	11	NULL	NULL	NULL				bind			central armadillo repeat region		cadherin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_23_16_6567_s_3	12878698	A deletion mutant betacatdeltaARM consists of the N- and  C-terminal domains of wild-type beta-catenin that contain, respectively,  alpha-catenin and postsynaptic density-95 (PSD-95)/discs large (Dlg)/zona  occludens-1 (ZO-1) (PDZ) binding sites but lacks the central armadillo repeat  region that binds cadherins and other proteins.	bind
41981	1	9916	7	11	NULL	NULL	NULL	 			binds			central armadillo repeat region		cadherins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_23_16_6567_s_3	12878698	A deletion mutant betacatdeltaARM consists of the N- and  C-terminal domains of wild-type beta-catenin that contain, respectively,  alpha-catenin and postsynaptic density-95 (PSD-95)/discs large (Dlg)/zona  occludens-1 (ZO-1) (PDZ) binding sites but lacks the central armadillo repeat  region that binds cadherins and other proteins.	bind
34606	1	9919	6	11	NULL	NULL	NULL	c-Abl	GP	deletion mutant	does not bind					p53	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_3_741_s_6	10629029	A deletion mutant of c-Abl that does not bind to p53 is also incapable of activating p53 DNA binding.	bind
34607	2	9919	6	11	NULL	NULL	NULL	p53	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_3_741_s_6	10629029	A deletion mutant of c-Abl that does not bind to p53 is also incapable of activating p53 DNA binding.	bind
34608	3	9919	6	11	NULL	NULL	NULL	c-Abl	GP	deletion mutant	does not activate					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_3_741_s_6	10629029	A deletion mutant of c-Abl that does not bind to p53 is also incapable of activating p53 DNA binding.	bind
41985	1	9919	7	11	NULL	NULL	NULL	 c-Abl	GP	deletion mutant	does not bind					p53	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_3_741_s_6	10629029	A deletion mutant of c-Abl that does not bind to p53 is also incapable of activating p53 DNA binding.	bind
41986	2	9919	7	11	NULL	NULL	NULL	p53	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_3_741_s_6	10629029	A deletion mutant of c-Abl that does not bind to p53 is also incapable of activating p53 DNA binding.	bind
41987	3	9919	7	11	NULL	NULL	NULL	c-Abl	GP	deletion mutant	does not activate					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_3_741_s_6	10629029	A deletion mutant of c-Abl that does not bind to p53 is also incapable of activating p53 DNA binding.	bind
34601	1	9920	6	11	NULL	NULL	NULL	E4BdeltaU	GP		bind					VCP	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_659_s_143	14749733	A deletion mutant of E4B that  lacks the COOH-terminal U-box domain (E4BdeltaU) also bound to VCP, whereas a mutant that lacks the NH2-terminal domain (E4BdeltaN) did not.	bind
34602	2	9920	6	11	NULL	NULL	NULL	E4BdeltaN	GP		does not bind					VCP	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_659_s_143	14749733	A deletion mutant of E4B that  lacks the COOH-terminal U-box domain (E4BdeltaU) also bound to VCP, whereas a mutant that lacks the NH2-terminal domain (E4BdeltaN) did not.	bind
34603	3	9920	6	11	NULL	NULL	NULL	E4BdeltaU	GP		is					E4B that lacks the COOH-terminal U-box domain	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_659_s_143	14749733	A deletion mutant of E4B that  lacks the COOH-terminal U-box domain (E4BdeltaU) also bound to VCP, whereas a mutant that lacks the NH2-terminal domain (E4BdeltaN) did not.	bind
34604	4	9920	6	11	NULL	NULL	NULL	E4BdeltaN	GP		is					E4B that lacks the NH2-terminal domain	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_659_s_143	14749733	A deletion mutant of E4B that  lacks the COOH-terminal U-box domain (E4BdeltaU) also bound to VCP, whereas a mutant that lacks the NH2-terminal domain (E4BdeltaN) did not.	bind
41988	1	9920	7	11	NULL	NULL	NULL	E4BdeltaU	GP		is					E4B that lacks the COOH-terminal U-box domain	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_659_s_143	14749733	A deletion mutant of E4B that  lacks the COOH-terminal U-box domain (E4BdeltaU) also bound to VCP, whereas a mutant that lacks the NH2-terminal domain (E4BdeltaN) did not.	bind
41989	2	9920	7	11	NULL	NULL	NULL	E4BdeltaU	GP		bind					VCP	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_659_s_143	14749733	A deletion mutant of E4B that  lacks the COOH-terminal U-box domain (E4BdeltaU) also bound to VCP, whereas a mutant that lacks the NH2-terminal domain (E4BdeltaN) did not.	bind
41990	3	9920	7	11	NULL	NULL	NULL	E4BdeltaN	GP		is					E4B that lacks the NH2-terminal domain	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_659_s_143	14749733	A deletion mutant of E4B that  lacks the COOH-terminal U-box domain (E4BdeltaU) also bound to VCP, whereas a mutant that lacks the NH2-terminal domain (E4BdeltaN) did not.	bind
41991	4	9920	7	11	NULL	NULL	NULL	E4BdeltaN	GP		does not bind					VCP	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_659_s_143	14749733	A deletion mutant of E4B that  lacks the COOH-terminal U-box domain (E4BdeltaU) also bound to VCP, whereas a mutant that lacks the NH2-terminal domain (E4BdeltaN) did not.	bind
34724	1	9922	6	11	NULL	NULL	NULL	Dc 63	AminoAcid		does not bind					Ab P2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_3_525_s_192	10069801	A deletion mutant with a truncation of the C-terminal 63 amino acids (Dc 63) does not bind to Ab P2.	bind
49010	2	9922	6	11	NULL	NULL	NULL	Dc 63	AminoAcid		is					deletion mutant with truncation of C-terminal 63 amino acids	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_3_525_s_192	10069801	A deletion mutant with a truncation of the C-terminal 63 amino acids (Dc 63) does not bind to Ab P2.	bind
41993	1	9922	7	11	NULL	NULL	NULL	Dc 63	AminoAcid		does not bind					Ab P2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_3_525_s_192	10069801	A deletion mutant with a truncation of the C-terminal 63 amino acids (Dc 63) does not bind to Ab P2.	bind
41994	2	9922	7	11	NULL	NULL	NULL	Dc 63	AminoAcid		is					deletion mutant with truncation of C-terminal 63 amino acids	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_3_525_s_192	10069801	A deletion mutant with a truncation of the C-terminal 63 amino acids (Dc 63) does not bind to Ab P2.	bind
34725	1	9923	6	11	NULL	NULL	NULL	Ssdp1	GP	mouse;; deletion of	does not bind			amino acid residues 1 to 121		Ldb1	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_22_14320_s_126	12381786	A deletion of amino acid residues 1 to 121 from mouse Ssdp1 (see Fig.  1 B) yielded a protein that did not bind Ldb1 after cotransfection into cultured cells and was also unable to synergize with Xlim1 and Ldb1 in axis induction (data not shown).	bind
34726	2	9923	6	11	NULL	NULL	NULL	Xlim1	GP		plays a role in					axis 	Process	induction of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_22_14320_s_126	12381786	A deletion of amino acid residues 1 to 121 from mouse Ssdp1 (see Fig.  1 B) yielded a protein that did not bind Ldb1 after cotransfection into cultured cells and was also unable to synergize with Xlim1 and Ldb1 in axis induction (data not shown).	bind
34727	3	9923	6	11	NULL	NULL	NULL	Ldb1	GP		plays a role in					axis	Process	induction of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_22_14320_s_126	12381786	A deletion of amino acid residues 1 to 121 from mouse Ssdp1 (see Fig.  1 B) yielded a protein that did not bind Ldb1 after cotransfection into cultured cells and was also unable to synergize with Xlim1 and Ldb1 in axis induction (data not shown).	bind
34856	4	9923	6	11	NULL	NULL	NULL	Ssdp1	GP	mouse;; deletion of	does not synergize with			amino acid residues 1 to 121		Xlim1	GP				NULL	statement 2	NULL	NULL	NULL	NULL	gw60_pnas_99_22_14320_s_126	12381786	A deletion of amino acid residues 1 to 121 from mouse Ssdp1 (see Fig.  1 B) yielded a protein that did not bind Ldb1 after cotransfection into cultured cells and was also unable to synergize with Xlim1 and Ldb1 in axis induction (data not shown).	bind
34857	5	9923	6	11	NULL	NULL	NULL	Ssdp1	GP	mouse;; deletion of	does not synergize with			amino acid residues 1 to 121		Ldb1	GP				NULL	statement 3	NULL	NULL	NULL	NULL	gw60_pnas_99_22_14320_s_126	12381786	A deletion of amino acid residues 1 to 121 from mouse Ssdp1 (see Fig.  1 B) yielded a protein that did not bind Ldb1 after cotransfection into cultured cells and was also unable to synergize with Xlim1 and Ldb1 in axis induction (data not shown).	bind
41997	1	9923	7	11	NULL	NULL	NULL	Ssdp1	GP	mouse;;deletion of	does not bind			amino acid residues 1 to 121 		Ldb1	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_22_14320_s_126	12381786	A deletion of amino acid residues 1 to 121 from mouse Ssdp1 (see Fig.  1 B) yielded a protein that did not bind Ldb1 after cotransfection into cultured cells and was also unable to synergize with Xlim1 and Ldb1 in axis induction (data not shown).	bind
41998	2	9923	7	11	NULL	NULL	NULL	Xlim1	GP		plays a role in					axis	Process	induction of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_22_14320_s_126	12381786	A deletion of amino acid residues 1 to 121 from mouse Ssdp1 (see Fig.  1 B) yielded a protein that did not bind Ldb1 after cotransfection into cultured cells and was also unable to synergize with Xlim1 and Ldb1 in axis induction (data not shown).	bind
41999	3	9923	7	11	NULL	NULL	NULL	Ldb1	GP		plays a role in					axis	Process	induction of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_22_14320_s_126	12381786	A deletion of amino acid residues 1 to 121 from mouse Ssdp1 (see Fig.  1 B) yielded a protein that did not bind Ldb1 after cotransfection into cultured cells and was also unable to synergize with Xlim1 and Ldb1 in axis induction (data not shown).	bind
42000	4	9923	7	11	NULL	NULL	NULL	Ssdp1	GP	mouse;;deletion of	does not syngergize with			amino acid residues 1 to 121 		Xlim1	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_22_14320_s_126	12381786	A deletion of amino acid residues 1 to 121 from mouse Ssdp1 (see Fig.  1 B) yielded a protein that did not bind Ldb1 after cotransfection into cultured cells and was also unable to synergize with Xlim1 and Ldb1 in axis induction (data not shown).	bind
42001	5	9923	7	11	NULL	NULL	NULL	Ssdp1	GP	mouse;;deletion of	does not syngergize with			amino acid residues 1 to 121 		Ldb1	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_22_14320_s_126	12381786	A deletion of amino acid residues 1 to 121 from mouse Ssdp1 (see Fig.  1 B) yielded a protein that did not bind Ldb1 after cotransfection into cultured cells and was also unable to synergize with Xlim1 and Ldb1 in axis induction (data not shown).	bind
34858	1	9924	6	11	NULL	NULL	NULL			deletion of	plays a role in		may	delta140 - 142		RNA	NucleicAcid	binding of			NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_13_4368_s_188	16077031	A deletion of residues delta140 - 142 (RRE), which we suspected might play a role in RNA binding due to the similarity of this region with the RNA-binding motif of lambda N protein and HIV Tat, indeed abolished both binding of the L18:pre-5S complex ( Figure 5) and enzyme activity	bind
34859	2	9924	6	11	NULL	NULL	NULL	RRE	AminoAcid		is					residues delta140 - 142	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_13_4368_s_188	16077031	A deletion of residues delta140 - 142 (RRE), which we suspected might play a role in RNA binding due to the similarity of this region with the RNA-binding motif of lambda N protein and HIV Tat, indeed abolished both binding of the L18:pre-5S complex ( Figure 5) and enzyme activity	bind
34860	3	9924	6	11	NULL	NULL	NULL				is similar to			RRE		lambda N protein	GP		RNA binding motif		NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_13_4368_s_188	16077031	A deletion of residues delta140 - 142 (RRE), which we suspected might play a role in RNA binding due to the similarity of this region with the RNA-binding motif of lambda N protein and HIV Tat, indeed abolished both binding of the L18:pre-5S complex ( Figure 5) and enzyme activity	bind
34861	4	9924	6	11	NULL	NULL	NULL				is similar to			RRE		HIV Tat	GP		RNA-binding motif		NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_13_4368_s_188	16077031	A deletion of residues delta140 - 142 (RRE), which we suspected might play a role in RNA binding due to the similarity of this region with the RNA-binding motif of lambda N protein and HIV Tat, indeed abolished both binding of the L18:pre-5S complex ( Figure 5) and enzyme activity	bind
34862	5	9924	6	11	NULL	NULL	NULL				abolishes			RRE		L18:pre-5S complex	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_13_4368_s_188	16077031	A deletion of residues delta140 - 142 (RRE), which we suspected might play a role in RNA binding due to the similarity of this region with the RNA-binding motif of lambda N protein and HIV Tat, indeed abolished both binding of the L18:pre-5S complex ( Figure 5) and enzyme activity	bind
34863	6	9924	6	11	NULL	NULL	NULL				abolishes			RRE		enzyme	GP	activity of 			NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_13_4368_s_188	16077031	A deletion of residues delta140 - 142 (RRE), which we suspected might play a role in RNA binding due to the similarity of this region with the RNA-binding motif of lambda N protein and HIV Tat, indeed abolished both binding of the L18:pre-5S complex ( Figure 5) and enzyme activity	bind
42002	1	9924	7	11	NULL	NULL	NULL			deletion of	plays a role in			 delta140 - 142		RNA	NucleicAcid	binding of			NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_13_4368_s_188	16077031	A deletion of residues delta140 - 142 (RRE), which we suspected might play a role in RNA binding due to the similarity of this region with the RNA-binding motif of lambda N protein and HIV Tat, indeed abolished both binding of the L18:pre-5S complex ( Figure 5) and enzyme activity	bind
42003	2	9924	7	11	NULL	NULL	NULL				is similar to			delta140 - 142		lambda N protein	GP		RNA-binding motif		NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_13_4368_s_188	16077031	A deletion of residues delta140 - 142 (RRE), which we suspected might play a role in RNA binding due to the similarity of this region with the RNA-binding motif of lambda N protein and HIV Tat, indeed abolished both binding of the L18:pre-5S complex ( Figure 5) and enzyme activity	bind
42004	3	9924	7	11	NULL	NULL	NULL				is similar to			delta140 - 142		HIV Tat	GP		RNA-binding motif		NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_13_4368_s_188	16077031	A deletion of residues delta140 - 142 (RRE), which we suspected might play a role in RNA binding due to the similarity of this region with the RNA-binding motif of lambda N protein and HIV Tat, indeed abolished both binding of the L18:pre-5S complex ( Figure 5) and enzyme activity	bind
42005	4	9924	7	11	NULL	NULL	NULL				abolishes			delta140 - 142		L18:pre-5S complex	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_13_4368_s_188	16077031	A deletion of residues delta140 - 142 (RRE), which we suspected might play a role in RNA binding due to the similarity of this region with the RNA-binding motif of lambda N protein and HIV Tat, indeed abolished both binding of the L18:pre-5S complex ( Figure 5) and enzyme activity	bind
42006	5	9924	7	11	NULL	NULL	NULL				abolishes			delta140 - 142		enzyme	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_13_4368_s_188	16077031	A deletion of residues delta140 - 142 (RRE), which we suspected might play a role in RNA binding due to the similarity of this region with the RNA-binding motif of lambda N protein and HIV Tat, indeed abolished both binding of the L18:pre-5S complex ( Figure 5) and enzyme activity	bind
49814	6	9924	7	11	NULL	NULL	NULL	RRE	AminoAcid		is					residues delta140-142	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_13_4368_s_188	16077031	A deletion of residues delta140 - 142 (RRE), which we suspected might play a role in RNA binding due to the similarity of this region with the RNA-binding motif of lambda N protein and HIV Tat, indeed abolished both binding of the L18:pre-5S complex ( Figure 5) and enzyme activity	bind
34864	1	9925	6	11	NULL	NULL	NULL	pG180DS2	NucleicAcid		eliminates					preS	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_14_8382_s_211	9525948	A deletion of the second domain and the N-terminal half of the third domain (pG180DS2) eliminated preS binding but showed carboxypeptidase activity (Figs.  4 and  5).	bind
34865	2	9925	6	11	NULL	NULL	NULL	pG180DS2	NucleicAcid		shows					carboxypeptidase activity 	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_14_8382_s_211	9525948	A deletion of the second domain and the N-terminal half of the third domain (pG180DS2) eliminated preS binding but showed carboxypeptidase activity (Figs.  4 and  5).	bind
34866	3	9925	6	11	NULL	NULL	NULL	pG180DS2	NucleicAcid		is					deletion of the second domain and the N-terminal half of the third domain	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_14_8382_s_211	9525948	A deletion of the second domain and the N-terminal half of the third domain (pG180DS2) eliminated preS binding but showed carboxypeptidase activity (Figs.  4 and  5).	bind
42086	1	9925	7	11	NULL	NULL	NULL	pG180DS2	NucleicAcid		eliminates					preS	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_14_8382_s_211	9525948	A deletion of the second domain and the N-terminal half of the third domain (pG180DS2) eliminated preS binding but showed carboxypeptidase activity (Figs.  4 and  5).	bind
42087	2	9925	7	11	NULL	NULL	NULL	pG180DS2	NucleicAcid		shows 					carboxypeptidase activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_14_8382_s_211	9525948	A deletion of the second domain and the N-terminal half of the third domain (pG180DS2) eliminated preS binding but showed carboxypeptidase activity (Figs.  4 and  5).	bind
42088	3	9925	7	11	NULL	NULL	NULL	pG180DS2	NucleicAcid		is					deletion of the second domain and the N-terminal half of the third domain	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_14_8382_s_211	9525948	A deletion of the second domain and the N-terminal half of the third domain (pG180DS2) eliminated preS binding but showed carboxypeptidase activity (Figs.  4 and  5).	bind
34728	1	9926	6	11	NULL	NULL	NULL	PTEN	GP		bind					PDZ domain-containing proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_14_6211_s_43	15988030	A deltaPDZB mutant was created with 3' primers bearing TKV/TVD mutations to disrupt PTEN's binding to PDZ domain-containing proteins.	bind
34729	2	9926	6	11	NULL	NULL	NULL	deltaPDZB	GP	mutant	disrupts			TKV/TVD		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_14_6211_s_43	15988030	A deltaPDZB mutant was created with 3' primers bearing TKV/TVD mutations to disrupt PTEN's binding to PDZ domain-containing proteins.	bind
42089	1	9926	7	11	NULL	NULL	NULL	PTEN's	GP		bind					PDZ domain-containing proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_14_6211_s_43	15988030	A deltaPDZB mutant was created with 3' primers bearing TKV/TVD mutations to disrupt PTEN's binding to PDZ domain-containing proteins.	bind
42090	2	9926	7	11	NULL	NULL	NULL	deltaPDZB	GP	mutant	disrupts			TKV/TVD		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_14_6211_s_43	15988030	A deltaPDZB mutant was created with 3' primers bearing TKV/TVD mutations to disrupt PTEN's binding to PDZ domain-containing proteins.	bind
34730	1	9928	6	11	NULL	NULL	NULL	beta1D construct	GP		bind					talin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_11_6104_s_173	9497328	A densitometric analysis of the Coomassie Blue-stained proteins indicated that the beta1D construct bound 9 times more talin, and the beta7 construct bound 8.4 times more filamin than the beta1A model protein (Fig.  8).	bind
34731	2	9928	6	11	NULL	NULL	NULL	beta7 construct	GP		bind					filamin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_11_6104_s_173	9497328	A densitometric analysis of the Coomassie Blue-stained proteins indicated that the beta1D construct bound 9 times more talin, and the beta7 construct bound 8.4 times more filamin than the beta1A model protein (Fig.  8).	bind
34732	3	9928	6	11	NULL	NULL	NULL	beta1A model protein	GP		bind					filamin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_11_6104_s_173	9497328	A densitometric analysis of the Coomassie Blue-stained proteins indicated that the beta1D construct bound 9 times more talin, and the beta7 construct bound 8.4 times more filamin than the beta1A model protein (Fig.  8).	bind
34733	4	9928	6	11	NULL	NULL	NULL	statement 2	Process	affinity of	is more than					statement 3	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_11_6104_s_173	9497328	A densitometric analysis of the Coomassie Blue-stained proteins indicated that the beta1D construct bound 9 times more talin, and the beta7 construct bound 8.4 times more filamin than the beta1A model protein (Fig.  8).	bind
49011	5	9928	6	11	NULL	NULL	NULL	beta1A model protein	GP		bind					talin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_11_6104_s_173	9497328	A densitometric analysis of the Coomassie Blue-stained proteins indicated that the beta1D construct bound 9 times more talin, and the beta7 construct bound 8.4 times more filamin than the beta1A model protein (Fig.  8).	bind
49012	6	9928	6	11	NULL	NULL	NULL	statement 1	Process	affinity of	is more than					statement 5	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_11_6104_s_173	9497328	A densitometric analysis of the Coomassie Blue-stained proteins indicated that the beta1D construct bound 9 times more talin, and the beta7 construct bound 8.4 times more filamin than the beta1A model protein (Fig.  8).	bind
42093	1	9928	7	11	NULL	NULL	NULL	beta1D construct	GP		bind					talin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_11_6104_s_173	9497328	A densitometric analysis of the Coomassie Blue-stained proteins indicated that the beta1D construct bound 9 times more talin, and the beta7 construct bound 8.4 times more filamin than the beta1A model protein (Fig.  8).	bind
42094	2	9928	7	11	NULL	NULL	NULL	beta7 construct	GP		bind					filamin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_11_6104_s_173	9497328	A densitometric analysis of the Coomassie Blue-stained proteins indicated that the beta1D construct bound 9 times more talin, and the beta7 construct bound 8.4 times more filamin than the beta1A model protein (Fig.  8).	bind
42095	3	9928	7	11	NULL	NULL	NULL	beta1A model protein	GP		bind					talin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_11_6104_s_173	9497328	A densitometric analysis of the Coomassie Blue-stained proteins indicated that the beta1D construct bound 9 times more talin, and the beta7 construct bound 8.4 times more filamin than the beta1A model protein (Fig.  8).	bind
42096	4	9928	7	11	NULL	NULL	NULL	beta1A model protein	GP		bind					filamin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_11_6104_s_173	9497328	A densitometric analysis of the Coomassie Blue-stained proteins indicated that the beta1D construct bound 9 times more talin, and the beta7 construct bound 8.4 times more filamin than the beta1A model protein (Fig.  8).	bind
42097	5	9928	7	11	NULL	NULL	NULL	statement 1	Process	binding of	is more than					statement 3	Process	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_11_6104_s_173	9497328	A densitometric analysis of the Coomassie Blue-stained proteins indicated that the beta1D construct bound 9 times more talin, and the beta7 construct bound 8.4 times more filamin than the beta1A model protein (Fig.  8).	bind
42098	6	9928	7	11	NULL	NULL	NULL	statement 2	Process	binding of	is more than					statement 4	Process	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_11_6104_s_173	9497328	A densitometric analysis of the Coomassie Blue-stained proteins indicated that the beta1D construct bound 9 times more talin, and the beta7 construct bound 8.4 times more filamin than the beta1A model protein (Fig.  8).	bind
34734	1	9929	6	11	NULL	NULL	NULL	Miz-1	GP		bind					AdML	Organism			promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_16_18_5672_s_86	9312026	A derivative of the AdML promoter which contains a mutated start site (kind gift of B.Roeder) was poorly transactivated by Miz-1, suggesting that binding of Miz-1 to the AdML promoter is required for activation (Figure  3B).	bind
34735	2	9929	6	11	NULL	NULL	NULL	statement 1	Process		is required for					AdML	Organism	activation of		promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_16_18_5672_s_86	9312026	A derivative of the AdML promoter which contains a mutated start site (kind gift of B.Roeder) was poorly transactivated by Miz-1, suggesting that binding of Miz-1 to the AdML promoter is required for activation (Figure  3B).	bind
42099	1	9929	7	11	NULL	NULL	NULL	 Miz-1	GP		bind					AdML	Organism			promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_16_18_5672_s_86	9312026	A derivative of the AdML promoter which contains a mutated start site (kind gift of B.Roeder) was poorly transactivated by Miz-1, suggesting that binding of Miz-1 to the AdML promoter is required for activation (Figure  3B).	bind
42100	2	9929	7	11	NULL	NULL	NULL	statement 1	Process		is required for					AdML	Organism	activation of		promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_16_18_5672_s_86	9312026	A derivative of the AdML promoter which contains a mutated start site (kind gift of B.Roeder) was poorly transactivated by Miz-1, suggesting that binding of Miz-1 to the AdML promoter is required for activation (Figure  3B).	bind
34867	1	9930	6	11	NULL	NULL	NULL	Desrt polypeptide	GP	recombinant	bind			amino acids 255-451 including the ARID domain		oligonucleotide	NucleicAcid			(TAA)9 repeat 	NULL		NULL	NULL	NULL	NULL	gw60_genomeres_11_8_1327_s_31	11483573	A Desrt recombinant polypeptide spanning amino acids 255-451 including the ARID domain binds a (TAA)9 repeat oligonucleotide that can be competed in a dose-dependent manner with excess unlabeled oligonucleotide (Complex C1) (Fig.  2B).	bind
42102	1	9930	7	11	NULL	NULL	NULL	Desrt polypeptide	GP	recombinant	binds			spanning amino acids 255-451 including the ARID domain		oligonucleotide	NucleicAcid			(TAA)9 repeat 	NULL		NULL	NULL	NULL	NULL	gw60_genomeres_11_8_1327_s_31	11483573	A Desrt recombinant polypeptide spanning amino acids 255-451 including the ARID domain binds a (TAA)9 repeat oligonucleotide that can be competed in a dose-dependent manner with excess unlabeled oligonucleotide (Complex C1) (Fig.  2B).	bind
34736	1	9931	6	11	NULL	NULL	NULL	ATVA	GP	mutant	bind		normally		destruction box	XDRP1	GP				NULL	egg extracts	NULL	NULL	NULL	NULL	gw60_embo_18_18_5009_s_180	10487753	A destruction-box mutant ATVA bound to XDRP1 normally in egg extracts (lane 4).	bind
42105	1	9931	7	11	NULL	NULL	NULL	ATVA	GP	mutant	bind		normally		destruction-box	XDRP1	GP				NULL	egg extracts	NULL	NULL	NULL	NULL	gw60_embo_18_18_5009_s_180	10487753	A destruction-box mutant ATVA bound to XDRP1 normally in egg extracts (lane 4).	bind
34737	1	9932	6	11	NULL	NULL	NULL	JIP-1	GP		bind					apoER2	GP		tail		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_33_25616_s_118	10827173	A detailed account of the binding properties of JIP-1 and JIP-2 to the apoER2 tail and the importance of the alternatively spliced insert is given in the accompanying paper by Stockinger  et al. ( 38).	bind
34738	2	9932	6	11	NULL	NULL	NULL	JIP-2	GP		bind					apoER2	GP		tail		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_33_25616_s_118	10827173	A detailed account of the binding properties of JIP-1 and JIP-2 to the apoER2 tail and the importance of the alternatively spliced insert is given in the accompanying paper by Stockinger  et al. ( 38).	bind
42106	1	9932	7	11	NULL	NULL	NULL	 JIP-1	GP		bind					apoER2	GP		tail		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_33_25616_s_118	10827173	A detailed account of the binding properties of JIP-1 and JIP-2 to the apoER2 tail and the importance of the alternatively spliced insert is given in the accompanying paper by Stockinger  et al. ( 38).	bind
42107	2	9932	7	11	NULL	NULL	NULL	JIP-2	GP		bind					apoER2	GP		tail		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_33_25616_s_118	10827173	A detailed account of the binding properties of JIP-1 and JIP-2 to the apoER2 tail and the importance of the alternatively spliced insert is given in the accompanying paper by Stockinger  et al. ( 38).	bind
34739	1	9933	6	11	NULL	NULL	NULL	ATP	Chemical		bind					Hsp90	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_30_18608_s_211	9228028	A detailed analysis of ATP binding to Hsp90 seems to be required in comparison to Hsp70 to identify potential steps in the interaction with partner proteins and steroid receptors that may require ATP binding to Hsp90.	bind
34740	2	9933	6	11	NULL	NULL	NULL	ATP	Chemical		bind					Hsp70	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_30_18608_s_211	9228028	A detailed analysis of ATP binding to Hsp90 seems to be required in comparison to Hsp70 to identify potential steps in the interaction with partner proteins and steroid receptors that may require ATP binding to Hsp90.	bind
49015	3	9933	6	11	NULL	NULL	NULL	steroid receptors	GP		require		may			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_30_18608_s_211	9228028	A detailed analysis of ATP binding to Hsp90 seems to be required in comparison to Hsp70 to identify potential steps in the interaction with partner proteins and steroid receptors that may require ATP binding to Hsp90.	bind
42108	1	9933	7	11	NULL	NULL	NULL	ATP	Chemical		bind					Hsp90	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_30_18608_s_211	9228028	A detailed analysis of ATP binding to Hsp90 seems to be required in comparison to Hsp70 to identify potential steps in the interaction with partner proteins and steroid receptors that may require ATP binding to Hsp90.	bind
42109	2	9933	7	11	NULL	NULL	NULL	ATP	Chemical		bind					Hsp70	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_30_18608_s_211	9228028	A detailed analysis of ATP binding to Hsp90 seems to be required in comparison to Hsp70 to identify potential steps in the interaction with partner proteins and steroid receptors that may require ATP binding to Hsp90.	bind
42110	3	9933	7	11	NULL	NULL	NULL	steroid receptors	GP		require		may			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_30_18608_s_211	9228028	A detailed analysis of ATP binding to Hsp90 seems to be required in comparison to Hsp70 to identify potential steps in the interaction with partner proteins and steroid receptors that may require ATP binding to Hsp90.	bind
34741	1	9934	6	11	NULL	NULL	NULL	Munc13-1	GP		bind					synaptobrevin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2520_s_155	8999968	A detailed analysis of Munc13-1 immunoprecipitation experiments and cosedimentation assays showed that in addition to syntaxin, Munc13-1 also binds synaptobrevin, SNAP25, and to a lesser extent, synaptotagmin (Figs.  4,  5,  6).	bind
34742	2	9934	6	11	NULL	NULL	NULL	Munc13-1	GP		bind					Syntaxin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2520_s_155	8999968	A detailed analysis of Munc13-1 immunoprecipitation experiments and cosedimentation assays showed that in addition to syntaxin, Munc13-1 also binds synaptobrevin, SNAP25, and to a lesser extent, synaptotagmin (Figs.  4,  5,  6).	bind
34743	3	9934	6	11	NULL	NULL	NULL	Munc13-1	GP		bind					SNAP25	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2520_s_155	8999968	A detailed analysis of Munc13-1 immunoprecipitation experiments and cosedimentation assays showed that in addition to syntaxin, Munc13-1 also binds synaptobrevin, SNAP25, and to a lesser extent, synaptotagmin (Figs.  4,  5,  6).	bind
34744	4	9934	6	11	NULL	NULL	NULL	Munc13-1	GP		bind					synaptotagmin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2520_s_155	8999968	A detailed analysis of Munc13-1 immunoprecipitation experiments and cosedimentation assays showed that in addition to syntaxin, Munc13-1 also binds synaptobrevin, SNAP25, and to a lesser extent, synaptotagmin (Figs.  4,  5,  6).	bind
42111	1	9934	7	11	NULL	NULL	NULL	Munc13-1	GP		binds					syntaxin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2520_s_155	8999968	A detailed analysis of Munc13-1 immunoprecipitation experiments and cosedimentation assays showed that in addition to syntaxin, Munc13-1 also binds synaptobrevin, SNAP25, and to a lesser extent, synaptotagmin (Figs.  4,  5,  6).	bind
42112	2	9934	7	11	NULL	NULL	NULL	Munc13-1	GP		binds					synaptobrevin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2520_s_155	8999968	A detailed analysis of Munc13-1 immunoprecipitation experiments and cosedimentation assays showed that in addition to syntaxin, Munc13-1 also binds synaptobrevin, SNAP25, and to a lesser extent, synaptotagmin (Figs.  4,  5,  6).	bind
42114	3	9934	7	11	NULL	NULL	NULL	 Munc13-1 	GP		binds					SNAP25	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2520_s_155	8999968	A detailed analysis of Munc13-1 immunoprecipitation experiments and cosedimentation assays showed that in addition to syntaxin, Munc13-1 also binds synaptobrevin, SNAP25, and to a lesser extent, synaptotagmin (Figs.  4,  5,  6).	bind
42116	4	9934	7	11	NULL	NULL	NULL	Munc13-1	GP		binds					synaptotagmin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2520_s_155	8999968	A detailed analysis of Munc13-1 immunoprecipitation experiments and cosedimentation assays showed that in addition to syntaxin, Munc13-1 also binds synaptobrevin, SNAP25, and to a lesser extent, synaptotagmin (Figs.  4,  5,  6).	bind
34745	1	9935	6	11	NULL	NULL	NULL	NFAT factor	GP		bind					HIV-1 clade	Organism			enhancer	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_51_52949_s_337	15466412	A detailed analysis of the binding of the NFAT factor to the different HIV-1 clade enhancers was also undertaken.	bind
42121	1	9935	7	11	NULL	NULL	NULL	NFAT factor	GP		bind					HIV-1 clade 	Organism			enhancer	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_51_52949_s_337	15466412	A detailed analysis of the binding of the NFAT factor to the different HIV-1 clade enhancers was also undertaken.	bind
34934	2	9937	6	11	NULL	NULL	NULL	FAD	Chemical		accommodate		might	QR1 binding site		statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_7_3177_s_201	10706635	A detailed analysis of the FAD contacts suggests then the binding site of the human and mouse QR1 might accommodate a certain degree of bending of the isoalloxazine around its central axis; in these two enzymes, the shortest van der Waals contacts occur at the center of the isoallozaxine ring and relax to longer contacts toward the extremes.	bind
34936	1	9937	6	11	NULL	NULL	NULL	isoalloxazine	Chemical		bends around					central axis	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_7_3177_s_201	10706635	A detailed analysis of the FAD contacts suggests then the binding site of the human and mouse QR1 might accommodate a certain degree of bending of the isoalloxazine around its central axis; in these two enzymes, the shortest van der Waals contacts occur at the center of the isoallozaxine ring and relax to longer contacts toward the extremes.	bind
35093	3	9937	6	11	NULL	NULL	NULL	FAD	Chemical		bind					QR1	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_7_3177_s_201	10706635	A detailed analysis of the FAD contacts suggests then the binding site of the human and mouse QR1 might accommodate a certain degree of bending of the isoalloxazine around its central axis; in these two enzymes, the shortest van der Waals contacts occur at the center of the isoallozaxine ring and relax to longer contacts toward the extremes.	bind
35094	4	9937	6	11	NULL	NULL	NULL	FAD	Chemical		bind					QR1	GP	mouse			NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_7_3177_s_201	10706635	A detailed analysis of the FAD contacts suggests then the binding site of the human and mouse QR1 might accommodate a certain degree of bending of the isoalloxazine around its central axis; in these two enzymes, the shortest van der Waals contacts occur at the center of the isoallozaxine ring and relax to longer contacts toward the extremes.	bind
42130	1	9937	7	11	NULL	NULL	NULL	QR1	GP	 human	bind					FAD	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_7_3177_s_201	10706635	A detailed analysis of the FAD contacts suggests then the binding site of the human and mouse QR1 might accommodate a certain degree of bending of the isoalloxazine around its central axis; in these two enzymes, the shortest van der Waals contacts occur at the center of the isoallozaxine ring and relax to longer contacts toward the extremes.	bind
42132	2	9937	7	11	NULL	NULL	NULL	QR1	GP	mouse	bind					FAD	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_7_3177_s_201	10706635	A detailed analysis of the FAD contacts suggests then the binding site of the human and mouse QR1 might accommodate a certain degree of bending of the isoalloxazine around its central axis; in these two enzymes, the shortest van der Waals contacts occur at the center of the isoallozaxine ring and relax to longer contacts toward the extremes.	bind
42133	4	9937	7	11	NULL	NULL	NULL	FAD	Chemical		accomodate		might	QR1 binding site		statement 3	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_7_3177_s_201	10706635	A detailed analysis of the FAD contacts suggests then the binding site of the human and mouse QR1 might accommodate a certain degree of bending of the isoalloxazine around its central axis; in these two enzymes, the shortest van der Waals contacts occur at the center of the isoallozaxine ring and relax to longer contacts toward the extremes.	bind
49018	3	9937	7	11	NULL	NULL	NULL	isoallozaxine	Chemical		bends around					central axis	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_7_3177_s_201	10706635	A detailed analysis of the FAD contacts suggests then the binding site of the human and mouse QR1 might accommodate a certain degree of bending of the isoalloxazine around its central axis; in these two enzymes, the shortest van der Waals contacts occur at the center of the isoallozaxine ring and relax to longer contacts toward the extremes.	bind
34937	1	9938	6	11	NULL	NULL	NULL	T3R heterodimer	GP		bind					9- cis RXR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27919_s_26	8910392	A detailed analysis of the human ppTRH gene promoter recently demonstrated that both the binding of T3Rs as heterodimers with the 9- cis-retinoic acid receptors (RXR) to the element that contains a single TRE half-site located 60 bp upstream of the TSS and the binding of T3R monomers to the two TRE half-sites positioning downstream of the TSS were required to exhibit full-inhibition of the human ppTRH gene promoter by T3 ( 7).	bind
34938	2	9938	6	11	NULL	NULL	NULL	RXR	GP		is					9- cis-retinoic acid receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27919_s_26	8910392	A detailed analysis of the human ppTRH gene promoter recently demonstrated that both the binding of T3Rs as heterodimers with the 9- cis-retinoic acid receptors (RXR) to the element that contains a single TRE half-site located 60 bp upstream of the TSS and the binding of T3R monomers to the two TRE half-sites positioning downstream of the TSS were required to exhibit full-inhibition of the human ppTRH gene promoter by T3 ( 7).	bind
34939	3	9938	6	11	NULL	NULL	NULL	statement 1	GP		bind					statement 8	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27919_s_26	8910392	A detailed analysis of the human ppTRH gene promoter recently demonstrated that both the binding of T3Rs as heterodimers with the 9- cis-retinoic acid receptors (RXR) to the element that contains a single TRE half-site located 60 bp upstream of the TSS and the binding of T3R monomers to the two TRE half-sites positioning downstream of the TSS were required to exhibit full-inhibition of the human ppTRH gene promoter by T3 ( 7).	bind
34940	4	9938	6	11	NULL	NULL	NULL	T3R monomers	GP		bind					statement 9	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27919_s_26	8910392	A detailed analysis of the human ppTRH gene promoter recently demonstrated that both the binding of T3Rs as heterodimers with the 9- cis-retinoic acid receptors (RXR) to the element that contains a single TRE half-site located 60 bp upstream of the TSS and the binding of T3R monomers to the two TRE half-sites positioning downstream of the TSS were required to exhibit full-inhibition of the human ppTRH gene promoter by T3 ( 7).	bind
34941	5	9938	6	11	NULL	NULL	NULL	T3	GP		inhibit					ppTRH gene	GP	human		promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27919_s_26	8910392	A detailed analysis of the human ppTRH gene promoter recently demonstrated that both the binding of T3Rs as heterodimers with the 9- cis-retinoic acid receptors (RXR) to the element that contains a single TRE half-site located 60 bp upstream of the TSS and the binding of T3R monomers to the two TRE half-sites positioning downstream of the TSS were required to exhibit full-inhibition of the human ppTRH gene promoter by T3 ( 7).	bind
49016	6	9938	6	11	NULL	NULL	NULL	statement 3	Process		is required for					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27919_s_26	8910392	A detailed analysis of the human ppTRH gene promoter recently demonstrated that both the binding of T3Rs as heterodimers with the 9- cis-retinoic acid receptors (RXR) to the element that contains a single TRE half-site located 60 bp upstream of the TSS and the binding of T3R monomers to the two TRE half-sites positioning downstream of the TSS were required to exhibit full-inhibition of the human ppTRH gene promoter by T3 ( 7).	bind
49017	7	9938	6	11	NULL	NULL	NULL	statement 4	Process		is required for					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27919_s_26	8910392	A detailed analysis of the human ppTRH gene promoter recently demonstrated that both the binding of T3Rs as heterodimers with the 9- cis-retinoic acid receptors (RXR) to the element that contains a single TRE half-site located 60 bp upstream of the TSS and the binding of T3R monomers to the two TRE half-sites positioning downstream of the TSS were required to exhibit full-inhibition of the human ppTRH gene promoter by T3 ( 7).	bind
56927	8	9938	6	11	NULL	NULL	NULL				is located				TRE half site			upstream of		TSS	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27919_s_26	8910392	A detailed analysis of the human ppTRH gene promoter recently demonstrated that both the binding of T3Rs as heterodimers with the 9- cis-retinoic acid receptors (RXR) to the element that contains a single TRE half-site located 60 bp upstream of the TSS and the binding of T3R monomers to the two TRE half-sites positioning downstream of the TSS were required to exhibit full-inhibition of the human ppTRH gene promoter by T3 ( 7).	bind
56928	9	9938	6	11	NULL	NULL	NULL				is located				TRE half site			downstream of		TSS	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27919_s_26	8910392	A detailed analysis of the human ppTRH gene promoter recently demonstrated that both the binding of T3Rs as heterodimers with the 9- cis-retinoic acid receptors (RXR) to the element that contains a single TRE half-site located 60 bp upstream of the TSS and the binding of T3R monomers to the two TRE half-sites positioning downstream of the TSS were required to exhibit full-inhibition of the human ppTRH gene promoter by T3 ( 7).	bind
42135	1	9938	7	11	NULL	NULL	NULL	T3R heterodimer	GP		bind					RXR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27919_s_26	8910392	A detailed analysis of the human ppTRH gene promoter recently demonstrated that both the binding of T3Rs as heterodimers with the 9- cis-retinoic acid receptors (RXR) to the element that contains a single TRE half-site located 60 bp upstream of the TSS and the binding of T3R monomers to the two TRE half-sites positioning downstream of the TSS were required to exhibit full-inhibition of the human ppTRH gene promoter by T3 ( 7).	bind
42136	2	9938	7	11	NULL	NULL	NULL	statement 1	GP		bind					statement 8	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27919_s_26	8910392	A detailed analysis of the human ppTRH gene promoter recently demonstrated that both the binding of T3Rs as heterodimers with the 9- cis-retinoic acid receptors (RXR) to the element that contains a single TRE half-site located 60 bp upstream of the TSS and the binding of T3R monomers to the two TRE half-sites positioning downstream of the TSS were required to exhibit full-inhibition of the human ppTRH gene promoter by T3 ( 7).	bind
42137	3	9938	7	11	NULL	NULL	NULL	T3R monomer	GP		bind					statement 9	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27919_s_26	8910392	A detailed analysis of the human ppTRH gene promoter recently demonstrated that both the binding of T3Rs as heterodimers with the 9- cis-retinoic acid receptors (RXR) to the element that contains a single TRE half-site located 60 bp upstream of the TSS and the binding of T3R monomers to the two TRE half-sites positioning downstream of the TSS were required to exhibit full-inhibition of the human ppTRH gene promoter by T3 ( 7).	bind
42138	4	9938	7	11	NULL	NULL	NULL	T3	GP		inhibit					ppTRH gene	GP	human		promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27919_s_26	8910392	A detailed analysis of the human ppTRH gene promoter recently demonstrated that both the binding of T3Rs as heterodimers with the 9- cis-retinoic acid receptors (RXR) to the element that contains a single TRE half-site located 60 bp upstream of the TSS and the binding of T3R monomers to the two TRE half-sites positioning downstream of the TSS were required to exhibit full-inhibition of the human ppTRH gene promoter by T3 ( 7).	bind
42139	5	9938	7	11	NULL	NULL	NULL	statement 2	Process		is required for					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27919_s_26	8910392	A detailed analysis of the human ppTRH gene promoter recently demonstrated that both the binding of T3Rs as heterodimers with the 9- cis-retinoic acid receptors (RXR) to the element that contains a single TRE half-site located 60 bp upstream of the TSS and the binding of T3R monomers to the two TRE half-sites positioning downstream of the TSS were required to exhibit full-inhibition of the human ppTRH gene promoter by T3 ( 7).	bind
42140	6	9938	7	11	NULL	NULL	NULL	statement 3	Process		is required for					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27919_s_26	8910392	A detailed analysis of the human ppTRH gene promoter recently demonstrated that both the binding of T3Rs as heterodimers with the 9- cis-retinoic acid receptors (RXR) to the element that contains a single TRE half-site located 60 bp upstream of the TSS and the binding of T3R monomers to the two TRE half-sites positioning downstream of the TSS were required to exhibit full-inhibition of the human ppTRH gene promoter by T3 ( 7).	bind
42141	7	9938	7	11	NULL	NULL	NULL	RXR	GP		is					 9- cis-retinoic acid receptors 	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27919_s_26	8910392	A detailed analysis of the human ppTRH gene promoter recently demonstrated that both the binding of T3Rs as heterodimers with the 9- cis-retinoic acid receptors (RXR) to the element that contains a single TRE half-site located 60 bp upstream of the TSS and the binding of T3R monomers to the two TRE half-sites positioning downstream of the TSS were required to exhibit full-inhibition of the human ppTRH gene promoter by T3 ( 7).	bind
56929	8	9938	7	11	NULL	NULL	NULL				is located				TRE half site			upstream of		TSS	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27919_s_26	8910392	A detailed analysis of the human ppTRH gene promoter recently demonstrated that both the binding of T3Rs as heterodimers with the 9- cis-retinoic acid receptors (RXR) to the element that contains a single TRE half-site located 60 bp upstream of the TSS and the binding of T3R monomers to the two TRE half-sites positioning downstream of the TSS were required to exhibit full-inhibition of the human ppTRH gene promoter by T3 ( 7).	bind
56930	9	9938	7	11	NULL	NULL	NULL				is located				TRE half site			downstream of		TSS	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27919_s_26	8910392	A detailed analysis of the human ppTRH gene promoter recently demonstrated that both the binding of T3Rs as heterodimers with the 9- cis-retinoic acid receptors (RXR) to the element that contains a single TRE half-site located 60 bp upstream of the TSS and the binding of T3R monomers to the two TRE half-sites positioning downstream of the TSS were required to exhibit full-inhibition of the human ppTRH gene promoter by T3 ( 7).	bind
34748	1	9939	6	11	NULL	NULL	NULL	TBP	GP		bind					C7 variant	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_14623_s_149	11278275	A detailed analysis of the kinetics of TBP binding the C7 variant is in progress and will be published elsewhere.	bind
42142	1	9939	7	11	NULL	NULL	NULL	TBP	GP		bind					C7 variant	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_14623_s_149	11278275	A detailed analysis of the kinetics of TBP binding the C7 variant is in progress and will be published elsewhere.	bind
34749	1	9940	6	11	NULL	NULL	NULL	HSP90	GP		bind							isolated	CS domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_16_16511_s_154	14761955	A detailed analysis of the peaks that disappear in the spectra of intact Sgt1 upon binding of HSP90 reveals that these signals correspond very closely to those affected by binding of HSP90 to the isolated CS domain ( cf.  Fig. 1 B).	bind
49019	2	9940	6	11	NULL	NULL	NULL	HSP90	GP		bind					Sgt1	GP	intact			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_16_16511_s_154	14761955	A detailed analysis of the peaks that disappear in the spectra of intact Sgt1 upon binding of HSP90 reveals that these signals correspond very closely to those affected by binding of HSP90 to the isolated CS domain ( cf.  Fig. 1 B).	bind
42143	1	9940	7	11	NULL	NULL	NULL	HSP90	GP		bind					Sgt1	GP	intact			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_16_16511_s_154	14761955	A detailed analysis of the peaks that disappear in the spectra of intact Sgt1 upon binding of HSP90 reveals that these signals correspond very closely to those affected by binding of HSP90 to the isolated CS domain ( cf.  Fig. 1 B).	bind
42144	2	9940	7	11	NULL	NULL	NULL	HSP90	GP		bind							isolated	CS domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_16_16511_s_154	14761955	A detailed analysis of the peaks that disappear in the spectra of intact Sgt1 upon binding of HSP90 reveals that these signals correspond very closely to those affected by binding of HSP90 to the isolated CS domain ( cf.  Fig. 1 B).	bind
34942	1	9941	6	11	NULL	NULL	NULL	RBCS	GP		is  					ribulose 1,5-bisphosphate carboxylase small subunit	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5256_s_23	12954761	A detailed analysis of the promoter of some of these genes, such as ribulose 1,5-bisphosphate carboxylase small subunit ( RBCS) and nuclear-encoded photosynthesis related genes for chlorophyll a/b binding proteins ( CAB) revealed the presence of several light responsive elements (LREs), such as G, GATA, GT1 and Z-box that are critical for light-controlled transcriptional activity ( 23 -  28).	bind
34943	2	9941	6	11	NULL	NULL	NULL	CAB	GP		is					chlorophyll a/b binding proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5256_s_23	12954761	A detailed analysis of the promoter of some of these genes, such as ribulose 1,5-bisphosphate carboxylase small subunit ( RBCS) and nuclear-encoded photosynthesis related genes for chlorophyll a/b binding proteins ( CAB) revealed the presence of several light responsive elements (LREs), such as G, GATA, GT1 and Z-box that are critical for light-controlled transcriptional activity ( 23 -  28).	bind
34944	3	9941	6	11	NULL	NULL	NULL	LRE	GP		is					light responsive elements	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5256_s_23	12954761	A detailed analysis of the promoter of some of these genes, such as ribulose 1,5-bisphosphate carboxylase small subunit ( RBCS) and nuclear-encoded photosynthesis related genes for chlorophyll a/b binding proteins ( CAB) revealed the presence of several light responsive elements (LREs), such as G, GATA, GT1 and Z-box that are critical for light-controlled transcriptional activity ( 23 -  28).	bind
34945	4	9941	6	11	NULL	NULL	NULL	G	GP		is a type of					LRE	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5256_s_23	12954761	A detailed analysis of the promoter of some of these genes, such as ribulose 1,5-bisphosphate carboxylase small subunit ( RBCS) and nuclear-encoded photosynthesis related genes for chlorophyll a/b binding proteins ( CAB) revealed the presence of several light responsive elements (LREs), such as G, GATA, GT1 and Z-box that are critical for light-controlled transcriptional activity ( 23 -  28).	bind
34946	5	9941	6	11	NULL	NULL	NULL	GATA	GP		is a type of					LRE	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5256_s_23	12954761	A detailed analysis of the promoter of some of these genes, such as ribulose 1,5-bisphosphate carboxylase small subunit ( RBCS) and nuclear-encoded photosynthesis related genes for chlorophyll a/b binding proteins ( CAB) revealed the presence of several light responsive elements (LREs), such as G, GATA, GT1 and Z-box that are critical for light-controlled transcriptional activity ( 23 -  28).	bind
34947	6	9941	6	11	NULL	NULL	NULL	GT1	GP		is a type of					LRE	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5256_s_23	12954761	A detailed analysis of the promoter of some of these genes, such as ribulose 1,5-bisphosphate carboxylase small subunit ( RBCS) and nuclear-encoded photosynthesis related genes for chlorophyll a/b binding proteins ( CAB) revealed the presence of several light responsive elements (LREs), such as G, GATA, GT1 and Z-box that are critical for light-controlled transcriptional activity ( 23 -  28).	bind
34948	7	9941	6	11	NULL	NULL	NULL	Z-box	GP		is a type of					LRE	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5256_s_23	12954761	A detailed analysis of the promoter of some of these genes, such as ribulose 1,5-bisphosphate carboxylase small subunit ( RBCS) and nuclear-encoded photosynthesis related genes for chlorophyll a/b binding proteins ( CAB) revealed the presence of several light responsive elements (LREs), such as G, GATA, GT1 and Z-box that are critical for light-controlled transcriptional activity ( 23 -  28).	bind
34949	8	9941	6	11	NULL	NULL	NULL	G	GP		is critical for					transcriptional activity	Process	light-controlled			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5256_s_23	12954761	A detailed analysis of the promoter of some of these genes, such as ribulose 1,5-bisphosphate carboxylase small subunit ( RBCS) and nuclear-encoded photosynthesis related genes for chlorophyll a/b binding proteins ( CAB) revealed the presence of several light responsive elements (LREs), such as G, GATA, GT1 and Z-box that are critical for light-controlled transcriptional activity ( 23 -  28).	bind
34950	9	9941	6	11	NULL	NULL	NULL	GATA	GP		is critical for					transcriptional activity	Process	light-controlled			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5256_s_23	12954761	A detailed analysis of the promoter of some of these genes, such as ribulose 1,5-bisphosphate carboxylase small subunit ( RBCS) and nuclear-encoded photosynthesis related genes for chlorophyll a/b binding proteins ( CAB) revealed the presence of several light responsive elements (LREs), such as G, GATA, GT1 and Z-box that are critical for light-controlled transcriptional activity ( 23 -  28).	bind
34951	10	9941	6	11	NULL	NULL	NULL	GT1	GP		is critical for					transcriptional activity	Process	light-controlled			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5256_s_23	12954761	A detailed analysis of the promoter of some of these genes, such as ribulose 1,5-bisphosphate carboxylase small subunit ( RBCS) and nuclear-encoded photosynthesis related genes for chlorophyll a/b binding proteins ( CAB) revealed the presence of several light responsive elements (LREs), such as G, GATA, GT1 and Z-box that are critical for light-controlled transcriptional activity ( 23 -  28).	bind
34952	11	9941	6	11	NULL	NULL	NULL	Z-box	GP		is critical for					transcriptional activity	Process	light-controlled			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5256_s_23	12954761	A detailed analysis of the promoter of some of these genes, such as ribulose 1,5-bisphosphate carboxylase small subunit ( RBCS) and nuclear-encoded photosynthesis related genes for chlorophyll a/b binding proteins ( CAB) revealed the presence of several light responsive elements (LREs), such as G, GATA, GT1 and Z-box that are critical for light-controlled transcriptional activity ( 23 -  28).	bind
42145	1	9941	7	11	NULL	NULL	NULL	RBCS gene	GP		contains									G	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5256_s_23	12954761	A detailed analysis of the promoter of some of these genes, such as ribulose 1,5-bisphosphate carboxylase small subunit ( RBCS) and nuclear-encoded photosynthesis related genes for chlorophyll a/b binding proteins ( CAB) revealed the presence of several light responsive elements (LREs), such as G, GATA, GT1 and Z-box that are critical for light-controlled transcriptional activity ( 23 -  28).	bind
42146	2	9941	7	11	NULL	NULL	NULL	RBCS gene	GP		contains									GATA	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5256_s_23	12954761	A detailed analysis of the promoter of some of these genes, such as ribulose 1,5-bisphosphate carboxylase small subunit ( RBCS) and nuclear-encoded photosynthesis related genes for chlorophyll a/b binding proteins ( CAB) revealed the presence of several light responsive elements (LREs), such as G, GATA, GT1 and Z-box that are critical for light-controlled transcriptional activity ( 23 -  28).	bind
42147	3	9941	7	11	NULL	NULL	NULL	RBCS gene	GP		contains									GT1	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5256_s_23	12954761	A detailed analysis of the promoter of some of these genes, such as ribulose 1,5-bisphosphate carboxylase small subunit ( RBCS) and nuclear-encoded photosynthesis related genes for chlorophyll a/b binding proteins ( CAB) revealed the presence of several light responsive elements (LREs), such as G, GATA, GT1 and Z-box that are critical for light-controlled transcriptional activity ( 23 -  28).	bind
42148	4	9941	7	11	NULL	NULL	NULL	RBCS gene	GP		contains									Z-box	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5256_s_23	12954761	A detailed analysis of the promoter of some of these genes, such as ribulose 1,5-bisphosphate carboxylase small subunit ( RBCS) and nuclear-encoded photosynthesis related genes for chlorophyll a/b binding proteins ( CAB) revealed the presence of several light responsive elements (LREs), such as G, GATA, GT1 and Z-box that are critical for light-controlled transcriptional activity ( 23 -  28).	bind
42149	5	9941	7	11	NULL	NULL	NULL	CAB gene	GP		contains									G	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5256_s_23	12954761	A detailed analysis of the promoter of some of these genes, such as ribulose 1,5-bisphosphate carboxylase small subunit ( RBCS) and nuclear-encoded photosynthesis related genes for chlorophyll a/b binding proteins ( CAB) revealed the presence of several light responsive elements (LREs), such as G, GATA, GT1 and Z-box that are critical for light-controlled transcriptional activity ( 23 -  28).	bind
42150	6	9941	7	11	NULL	NULL	NULL	CAB gene	GP		contains									GATA	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5256_s_23	12954761	A detailed analysis of the promoter of some of these genes, such as ribulose 1,5-bisphosphate carboxylase small subunit ( RBCS) and nuclear-encoded photosynthesis related genes for chlorophyll a/b binding proteins ( CAB) revealed the presence of several light responsive elements (LREs), such as G, GATA, GT1 and Z-box that are critical for light-controlled transcriptional activity ( 23 -  28).	bind
42151	7	9941	7	11	NULL	NULL	NULL	CAB gene	GP		contains									GT1	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5256_s_23	12954761	A detailed analysis of the promoter of some of these genes, such as ribulose 1,5-bisphosphate carboxylase small subunit ( RBCS) and nuclear-encoded photosynthesis related genes for chlorophyll a/b binding proteins ( CAB) revealed the presence of several light responsive elements (LREs), such as G, GATA, GT1 and Z-box that are critical for light-controlled transcriptional activity ( 23 -  28).	bind
42152	8	9941	7	11	NULL	NULL	NULL	CAB gene	GP		contains									Z-box	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5256_s_23	12954761	A detailed analysis of the promoter of some of these genes, such as ribulose 1,5-bisphosphate carboxylase small subunit ( RBCS) and nuclear-encoded photosynthesis related genes for chlorophyll a/b binding proteins ( CAB) revealed the presence of several light responsive elements (LREs), such as G, GATA, GT1 and Z-box that are critical for light-controlled transcriptional activity ( 23 -  28).	bind
42153	9	9941	7	11	NULL	NULL	NULL	G	GP		is a type of					LREs	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5256_s_23	12954761	A detailed analysis of the promoter of some of these genes, such as ribulose 1,5-bisphosphate carboxylase small subunit ( RBCS) and nuclear-encoded photosynthesis related genes for chlorophyll a/b binding proteins ( CAB) revealed the presence of several light responsive elements (LREs), such as G, GATA, GT1 and Z-box that are critical for light-controlled transcriptional activity ( 23 -  28).	bind
42154	10	9941	7	11	NULL	NULL	NULL	GATA	GP		is a type of					LREs	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5256_s_23	12954761	A detailed analysis of the promoter of some of these genes, such as ribulose 1,5-bisphosphate carboxylase small subunit ( RBCS) and nuclear-encoded photosynthesis related genes for chlorophyll a/b binding proteins ( CAB) revealed the presence of several light responsive elements (LREs), such as G, GATA, GT1 and Z-box that are critical for light-controlled transcriptional activity ( 23 -  28).	bind
42155	11	9941	7	11	NULL	NULL	NULL	GT1	GP		is a type of					LREs	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5256_s_23	12954761	A detailed analysis of the promoter of some of these genes, such as ribulose 1,5-bisphosphate carboxylase small subunit ( RBCS) and nuclear-encoded photosynthesis related genes for chlorophyll a/b binding proteins ( CAB) revealed the presence of several light responsive elements (LREs), such as G, GATA, GT1 and Z-box that are critical for light-controlled transcriptional activity ( 23 -  28).	bind
42156	12	9941	7	11	NULL	NULL	NULL	Z-box	GP		is a type of					LREs	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5256_s_23	12954761	A detailed analysis of the promoter of some of these genes, such as ribulose 1,5-bisphosphate carboxylase small subunit ( RBCS) and nuclear-encoded photosynthesis related genes for chlorophyll a/b binding proteins ( CAB) revealed the presence of several light responsive elements (LREs), such as G, GATA, GT1 and Z-box that are critical for light-controlled transcriptional activity ( 23 -  28).	bind
42157	13	9941	7	11	NULL	NULL	NULL	RBCS	GP		is					ribulose 1,5-bisphosphate carboxylase small subunit	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5256_s_23	12954761	A detailed analysis of the promoter of some of these genes, such as ribulose 1,5-bisphosphate carboxylase small subunit ( RBCS) and nuclear-encoded photosynthesis related genes for chlorophyll a/b binding proteins ( CAB) revealed the presence of several light responsive elements (LREs), such as G, GATA, GT1 and Z-box that are critical for light-controlled transcriptional activity ( 23 -  28).	bind
42158	14	9941	7	11	NULL	NULL	NULL	CAB	GP		is					chlorophyll a/b binding proteins 	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5256_s_23	12954761	A detailed analysis of the promoter of some of these genes, such as ribulose 1,5-bisphosphate carboxylase small subunit ( RBCS) and nuclear-encoded photosynthesis related genes for chlorophyll a/b binding proteins ( CAB) revealed the presence of several light responsive elements (LREs), such as G, GATA, GT1 and Z-box that are critical for light-controlled transcriptional activity ( 23 -  28).	bind
42159	15	9941	7	11	NULL	NULL	NULL	CAB	GP		is a type of					nuclear-encoded photosynthesis related genes	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5256_s_23	12954761	A detailed analysis of the promoter of some of these genes, such as ribulose 1,5-bisphosphate carboxylase small subunit ( RBCS) and nuclear-encoded photosynthesis related genes for chlorophyll a/b binding proteins ( CAB) revealed the presence of several light responsive elements (LREs), such as G, GATA, GT1 and Z-box that are critical for light-controlled transcriptional activity ( 23 -  28).	bind
34750	1	9942	6	NULL	NULL	0	NULL	BaCRASP-1	NULL		bind	NULL	strongly			FHL-1/reconectin	NULL				NULL		0	NULL	NULL	NULL	abs-batch0600-0619_infect-immun_69_12_11705962_s_10	11705962	A detailed comparison  reveals overlapping and even identical binding profiles for BaCRASP-1  (27.5 kDa), BbCRASP-1 (25.9 kDa), and BbCRASP-2 (23.2 kDa), which bind  FHL-1/reconectin strongly and interact weakly with factor H.	bind
34751	2	9942	6	NULL	NULL	0	NULL	BbCRASP-1	NULL		bind	NULL	strongly			FHL-1/reconectin	NULL				NULL		0	NULL	NULL	NULL	abs-batch0600-0619_infect-immun_69_12_11705962_s_10	11705962	A detailed comparison  reveals overlapping and even identical binding profiles for BaCRASP-1  (27.5 kDa), BbCRASP-1 (25.9 kDa), and BbCRASP-2 (23.2 kDa), which bind  FHL-1/reconectin strongly and interact weakly with factor H.	bind
34752	3	9942	6	NULL	NULL	0	NULL	BbCRASP-2	NULL		bind	NULL	strongly			FHL-1/reconectin	NULL				NULL		0	NULL	NULL	NULL	abs-batch0600-0619_infect-immun_69_12_11705962_s_10	11705962	A detailed comparison  reveals overlapping and even identical binding profiles for BaCRASP-1  (27.5 kDa), BbCRASP-1 (25.9 kDa), and BbCRASP-2 (23.2 kDa), which bind  FHL-1/reconectin strongly and interact weakly with factor H.	bind
34753	4	9942	6	10	NULL	0	NULL	BaCRASP-1	NULL		interacts with	NULL	weakly 			factor H	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_infect-immun_69_12_11705962_s_10	11705962	A detailed comparison  reveals overlapping and even identical binding profiles for BaCRASP-1  (27.5 kDa), BbCRASP-1 (25.9 kDa), and BbCRASP-2 (23.2 kDa), which bind  FHL-1/reconectin strongly and interact weakly with factor H.	bind
34754	5	9942	6	10	NULL	0	NULL	BbCRASP-1	NULL		interacts with	NULL	weakly			factor H	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_infect-immun_69_12_11705962_s_10	11705962	A detailed comparison  reveals overlapping and even identical binding profiles for BaCRASP-1  (27.5 kDa), BbCRASP-1 (25.9 kDa), and BbCRASP-2 (23.2 kDa), which bind  FHL-1/reconectin strongly and interact weakly with factor H.	bind
34755	6	9942	6	10	NULL	0	NULL	BbCRASP-2	NULL		interacts with	NULL	weakly			factor H	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_infect-immun_69_12_11705962_s_10	11705962	A detailed comparison  reveals overlapping and even identical binding profiles for BaCRASP-1  (27.5 kDa), BbCRASP-1 (25.9 kDa), and BbCRASP-2 (23.2 kDa), which bind  FHL-1/reconectin strongly and interact weakly with factor H.	bind
42160	1	9942	7	NULL	NULL	0	NULL	BaCRASP-1 	NULL		bind	NULL	strongly			FHL-1/reconectin 	NULL				NULL		0	NULL	NULL	NULL	abs-batch0600-0619_infect-immun_69_12_11705962_s_10	11705962	A detailed comparison  reveals overlapping and even identical binding profiles for BaCRASP-1  (27.5 kDa), BbCRASP-1 (25.9 kDa), and BbCRASP-2 (23.2 kDa), which bind  FHL-1/reconectin strongly and interact weakly with factor H.	bind
42161	2	9942	7	NULL	NULL	0	NULL	BbCRASP-1	NULL		bind	NULL	strongly			FHL-1/reconectin 	NULL				NULL		0	NULL	NULL	NULL	abs-batch0600-0619_infect-immun_69_12_11705962_s_10	11705962	A detailed comparison  reveals overlapping and even identical binding profiles for BaCRASP-1  (27.5 kDa), BbCRASP-1 (25.9 kDa), and BbCRASP-2 (23.2 kDa), which bind  FHL-1/reconectin strongly and interact weakly with factor H.	bind
42162	3	9942	7	NULL	NULL	0	NULL	 BbCRASP-2 	NULL		bind	NULL	strongly			FHL-1/reconectin 	NULL				NULL		0	NULL	NULL	NULL	abs-batch0600-0619_infect-immun_69_12_11705962_s_10	11705962	A detailed comparison  reveals overlapping and even identical binding profiles for BaCRASP-1  (27.5 kDa), BbCRASP-1 (25.9 kDa), and BbCRASP-2 (23.2 kDa), which bind  FHL-1/reconectin strongly and interact weakly with factor H.	bind
42163	4	9942	7	10	NULL	0	NULL	BaCRASP-1	NULL		interacts with	NULL	weakly			factor H	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_infect-immun_69_12_11705962_s_10	11705962	A detailed comparison  reveals overlapping and even identical binding profiles for BaCRASP-1  (27.5 kDa), BbCRASP-1 (25.9 kDa), and BbCRASP-2 (23.2 kDa), which bind  FHL-1/reconectin strongly and interact weakly with factor H.	bind
42164	5	9942	7	10	NULL	0	NULL	BbCRASP-1	NULL		interacts with	NULL	weakly			factor H	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_infect-immun_69_12_11705962_s_10	11705962	A detailed comparison  reveals overlapping and even identical binding profiles for BaCRASP-1  (27.5 kDa), BbCRASP-1 (25.9 kDa), and BbCRASP-2 (23.2 kDa), which bind  FHL-1/reconectin strongly and interact weakly with factor H.	bind
42165	6	9942	7	10	NULL	0	NULL	BbCRASP-2	NULL		interacts with	NULL	weakly			factor H	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_infect-immun_69_12_11705962_s_10	11705962	A detailed comparison  reveals overlapping and even identical binding profiles for BaCRASP-1  (27.5 kDa), BbCRASP-1 (25.9 kDa), and BbCRASP-2 (23.2 kDa), which bind  FHL-1/reconectin strongly and interact weakly with factor H.	bind
34757	1	9944	6	11	NULL	NULL	NULL	c-Cbl	GP		bind					E2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_17_15341_s_268	12588869	A detailed comparison of the free EL5 RING finger domain with the E2-bound form of c-Cbl suggested that the side-chain conformations (chi1) of the Trp residues in both molecules are different (Fig.  3).	bind
42168	1	9944	7	11	NULL	NULL	NULL	E2	GP		bind					c-Cbl	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_17_15341_s_268	12588869	A detailed comparison of the free EL5 RING finger domain with the E2-bound form of c-Cbl suggested that the side-chain conformations (chi1) of the Trp residues in both molecules are different (Fig.  3).	bind
42169	2	9944	7	11	NULL	NULL	NULL	free EL5	GP	side-chain conformations of	differs from			Trp residues in RING finger domain		statement 1	GP	side-chain conformations of	Trp residues		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_17_15341_s_268	12588869	A detailed comparison of the free EL5 RING finger domain with the E2-bound form of c-Cbl suggested that the side-chain conformations (chi1) of the Trp residues in both molecules are different (Fig.  3).	bind
34758	1	9945	6	11	NULL	NULL	NULL	TIMP-2	GP		bind					N-MMP-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_34_21736_s_7	9705310	A detailed comparison of the N-TIMP-2 structure with that of TIMP-1 bound to N-MMP-3 (Gomis-Ruth, F.-X., Maskos, K., Betz, M., Bergner, A., Huber, R., Suzuki, K., Yoshida, N., Nagase, H., Brew, K., Bourne, G. P., Bartunik, H. & Bode, W. (1997)  Nature 389, 77-80) revealed that the core beta-barrels are very similar in topology but that the loop connecting beta-strands CD (P67-C72) would need to undergo a large conformational change for TIMP-2 to bind in a similar manner to TIMP-1.	bind
49670	2	9945	6	11	NULL	NULL	NULL	TIMP-1	GP		bind					N-MMP-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_34_21736_s_7	9705310	A detailed comparison of the N-TIMP-2 structure with that of TIMP-1 bound to N-MMP-3 (Gomis-Ruth, F.-X., Maskos, K., Betz, M., Bergner, A., Huber, R., Suzuki, K., Yoshida, N., Nagase, H., Brew, K., Bourne, G. P., Bartunik, H. & Bode, W. (1997)  Nature 389, 77-80) revealed that the core beta-barrels are very similar in topology but that the loop connecting beta-strands CD (P67-C72) would need to undergo a large conformational change for TIMP-2 to bind in a similar manner to TIMP-1.	bind
49671	3	9945	6	11	NULL	NULL	NULL	TIMP-1	GP		is similar to			core beta-barrels		TIMP-2	GP		core beta-barrels		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_34_21736_s_7	9705310	A detailed comparison of the N-TIMP-2 structure with that of TIMP-1 bound to N-MMP-3 (Gomis-Ruth, F.-X., Maskos, K., Betz, M., Bergner, A., Huber, R., Suzuki, K., Yoshida, N., Nagase, H., Brew, K., Bourne, G. P., Bartunik, H. & Bode, W. (1997)  Nature 389, 77-80) revealed that the core beta-barrels are very similar in topology but that the loop connecting beta-strands CD (P67-C72) would need to undergo a large conformational change for TIMP-2 to bind in a similar manner to TIMP-1.	bind
42170	1	9945	7	11	NULL	NULL	NULL	 TIMP-1	GP		bind					N-MMP-3 	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_34_21736_s_7	9705310	A detailed comparison of the N-TIMP-2 structure with that of TIMP-1 bound to N-MMP-3 (Gomis-Ruth, F.-X., Maskos, K., Betz, M., Bergner, A., Huber, R., Suzuki, K., Yoshida, N., Nagase, H., Brew, K., Bourne, G. P., Bartunik, H. & Bode, W. (1997)  Nature 389, 77-80) revealed that the core beta-barrels are very similar in topology but that the loop connecting beta-strands CD (P67-C72) would need to undergo a large conformational change for TIMP-2 to bind in a similar manner to TIMP-1.	bind
42171	2	9945	7	11	NULL	NULL	NULL	TIMP-2	GP		bind					N-MMP-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_34_21736_s_7	9705310	A detailed comparison of the N-TIMP-2 structure with that of TIMP-1 bound to N-MMP-3 (Gomis-Ruth, F.-X., Maskos, K., Betz, M., Bergner, A., Huber, R., Suzuki, K., Yoshida, N., Nagase, H., Brew, K., Bourne, G. P., Bartunik, H. & Bode, W. (1997)  Nature 389, 77-80) revealed that the core beta-barrels are very similar in topology but that the loop connecting beta-strands CD (P67-C72) would need to undergo a large conformational change for TIMP-2 to bind in a similar manner to TIMP-1.	bind
42172	3	9945	7	11	NULL	NULL	NULL	TIMP-1	GP		is similar to			core beta-barrels		N-TIMP-2	GP		core beta-barrels		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_34_21736_s_7	9705310	A detailed comparison of the N-TIMP-2 structure with that of TIMP-1 bound to N-MMP-3 (Gomis-Ruth, F.-X., Maskos, K., Betz, M., Bergner, A., Huber, R., Suzuki, K., Yoshida, N., Nagase, H., Brew, K., Bourne, G. P., Bartunik, H. & Bode, W. (1997)  Nature 389, 77-80) revealed that the core beta-barrels are very similar in topology but that the loop connecting beta-strands CD (P67-C72) would need to undergo a large conformational change for TIMP-2 to bind in a similar manner to TIMP-1.	bind
34953	1	9947	6	11	NULL	NULL	NULL	N-Oct-3	GP		bind			POU domain		AADC	GP	neuronal		promoter	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_5_1513_s_35	15767276	A detailed compilation of the available POU/DNA complex structures, as well as a combination of molecular modeling, DNA footprinting and electrophoretic mobility shift assay (EMSA) have enabled us to (i) uncover a new mode of homodimerization adopted by the N-Oct-3 POU domain bound to the respective neuronal AADC and CRH gene promoters, (ii) demonstrate that this pattern is induced by a novel structural motif, the NORE (N-Oct-3 responsive element) and (iii) understand how the same structural motif can also induce the formation of a heterodimer in association with HNF-3beta DBD.	bind
34954	2	9947	6	11	NULL	NULL	NULL	N-Oct-3	GP		bind			POU domain		CRH 	GP	neuronal		promoter	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_5_1513_s_35	15767276	A detailed compilation of the available POU/DNA complex structures, as well as a combination of molecular modeling, DNA footprinting and electrophoretic mobility shift assay (EMSA) have enabled us to (i) uncover a new mode of homodimerization adopted by the N-Oct-3 POU domain bound to the respective neuronal AADC and CRH gene promoters, (ii) demonstrate that this pattern is induced by a novel structural motif, the NORE (N-Oct-3 responsive element) and (iii) understand how the same structural motif can also induce the formation of a heterodimer in association with HNF-3beta DBD.	bind
34955	3	9947	6	11	NULL	NULL	NULL	NORE	GP		is					N-Oct-3 responsive element	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_5_1513_s_35	15767276	A detailed compilation of the available POU/DNA complex structures, as well as a combination of molecular modeling, DNA footprinting and electrophoretic mobility shift assay (EMSA) have enabled us to (i) uncover a new mode of homodimerization adopted by the N-Oct-3 POU domain bound to the respective neuronal AADC and CRH gene promoters, (ii) demonstrate that this pattern is induced by a novel structural motif, the NORE (N-Oct-3 responsive element) and (iii) understand how the same structural motif can also induce the formation of a heterodimer in association with HNF-3beta DBD.	bind
35095	4	9947	6	11	NULL	NULL	NULL	statement 1	GP		undergoes					homodimerization	Process				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_5_1513_s_35	15767276	A detailed compilation of the available POU/DNA complex structures, as well as a combination of molecular modeling, DNA footprinting and electrophoretic mobility shift assay (EMSA) have enabled us to (i) uncover a new mode of homodimerization adopted by the N-Oct-3 POU domain bound to the respective neuronal AADC and CRH gene promoters, (ii) demonstrate that this pattern is induced by a novel structural motif, the NORE (N-Oct-3 responsive element) and (iii) understand how the same structural motif can also induce the formation of a heterodimer in association with HNF-3beta DBD.	bind
35096	5	9947	6	11	NULL	NULL	NULL	statement 2	GP		undergoes					homodimerization	Process				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_5_1513_s_35	15767276	A detailed compilation of the available POU/DNA complex structures, as well as a combination of molecular modeling, DNA footprinting and electrophoretic mobility shift assay (EMSA) have enabled us to (i) uncover a new mode of homodimerization adopted by the N-Oct-3 POU domain bound to the respective neuronal AADC and CRH gene promoters, (ii) demonstrate that this pattern is induced by a novel structural motif, the NORE (N-Oct-3 responsive element) and (iii) understand how the same structural motif can also induce the formation of a heterodimer in association with HNF-3beta DBD.	bind
35097	6	9947	6	11	NULL	NULL	NULL	statement 4	Process		is induced by									NORE	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_5_1513_s_35	15767276	A detailed compilation of the available POU/DNA complex structures, as well as a combination of molecular modeling, DNA footprinting and electrophoretic mobility shift assay (EMSA) have enabled us to (i) uncover a new mode of homodimerization adopted by the N-Oct-3 POU domain bound to the respective neuronal AADC and CRH gene promoters, (ii) demonstrate that this pattern is induced by a novel structural motif, the NORE (N-Oct-3 responsive element) and (iii) understand how the same structural motif can also induce the formation of a heterodimer in association with HNF-3beta DBD.	bind
35098	7	9947	6	11	NULL	NULL	NULL	statement 5	Process		is induced by									NORE	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_5_1513_s_35	15767276	A detailed compilation of the available POU/DNA complex structures, as well as a combination of molecular modeling, DNA footprinting and electrophoretic mobility shift assay (EMSA) have enabled us to (i) uncover a new mode of homodimerization adopted by the N-Oct-3 POU domain bound to the respective neuronal AADC and CRH gene promoters, (ii) demonstrate that this pattern is induced by a novel structural motif, the NORE (N-Oct-3 responsive element) and (iii) understand how the same structural motif can also induce the formation of a heterodimer in association with HNF-3beta DBD.	bind
35099	8	9947	6	11	NULL	NULL	NULL	N-Oct-3	GP		forms heterodimer with			POU domain		HNF-3 beta	GP		DBD		NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_5_1513_s_35	15767276	A detailed compilation of the available POU/DNA complex structures, as well as a combination of molecular modeling, DNA footprinting and electrophoretic mobility shift assay (EMSA) have enabled us to (i) uncover a new mode of homodimerization adopted by the N-Oct-3 POU domain bound to the respective neuronal AADC and CRH gene promoters, (ii) demonstrate that this pattern is induced by a novel structural motif, the NORE (N-Oct-3 responsive element) and (iii) understand how the same structural motif can also induce the formation of a heterodimer in association with HNF-3beta DBD.	bind
35100	9	9947	6	11	NULL	NULL	NULL	statement 8	Process		is induced by									NORE	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_5_1513_s_35	15767276	A detailed compilation of the available POU/DNA complex structures, as well as a combination of molecular modeling, DNA footprinting and electrophoretic mobility shift assay (EMSA) have enabled us to (i) uncover a new mode of homodimerization adopted by the N-Oct-3 POU domain bound to the respective neuronal AADC and CRH gene promoters, (ii) demonstrate that this pattern is induced by a novel structural motif, the NORE (N-Oct-3 responsive element) and (iii) understand how the same structural motif can also induce the formation of a heterodimer in association with HNF-3beta DBD.	bind
42177	1	9947	7	11	NULL	NULL	NULL	N-Oct-3	GP		bind			POU domain		AADC gene	GP	neuronal		promoter	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_5_1513_s_35	15767276	A detailed compilation of the available POU/DNA complex structures, as well as a combination of molecular modeling, DNA footprinting and electrophoretic mobility shift assay (EMSA) have enabled us to (i) uncover a new mode of homodimerization adopted by the N-Oct-3 POU domain bound to the respective neuronal AADC and CRH gene promoters, (ii) demonstrate that this pattern is induced by a novel structural motif, the NORE (N-Oct-3 responsive element) and (iii) understand how the same structural motif can also induce the formation of a heterodimer in association with HNF-3beta DBD.	bind
42178	2	9947	7	11	NULL	NULL	NULL	N-Oct-3	GP		bind			POU domain		CRH gene	GP	neuronal		promoter	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_5_1513_s_35	15767276	A detailed compilation of the available POU/DNA complex structures, as well as a combination of molecular modeling, DNA footprinting and electrophoretic mobility shift assay (EMSA) have enabled us to (i) uncover a new mode of homodimerization adopted by the N-Oct-3 POU domain bound to the respective neuronal AADC and CRH gene promoters, (ii) demonstrate that this pattern is induced by a novel structural motif, the NORE (N-Oct-3 responsive element) and (iii) understand how the same structural motif can also induce the formation of a heterodimer in association with HNF-3beta DBD.	bind
42179	3	9947	7	11	NULL	NULL	NULL	statement 1	Process		undergoes					homodimerization	Process				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_5_1513_s_35	15767276	A detailed compilation of the available POU/DNA complex structures, as well as a combination of molecular modeling, DNA footprinting and electrophoretic mobility shift assay (EMSA) have enabled us to (i) uncover a new mode of homodimerization adopted by the N-Oct-3 POU domain bound to the respective neuronal AADC and CRH gene promoters, (ii) demonstrate that this pattern is induced by a novel structural motif, the NORE (N-Oct-3 responsive element) and (iii) understand how the same structural motif can also induce the formation of a heterodimer in association with HNF-3beta DBD.	bind
42180	4	9947	7	11	NULL	NULL	NULL	statement 2	Process		undergoes					homodimerization	Process				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_5_1513_s_35	15767276	A detailed compilation of the available POU/DNA complex structures, as well as a combination of molecular modeling, DNA footprinting and electrophoretic mobility shift assay (EMSA) have enabled us to (i) uncover a new mode of homodimerization adopted by the N-Oct-3 POU domain bound to the respective neuronal AADC and CRH gene promoters, (ii) demonstrate that this pattern is induced by a novel structural motif, the NORE (N-Oct-3 responsive element) and (iii) understand how the same structural motif can also induce the formation of a heterodimer in association with HNF-3beta DBD.	bind
42181	5	9947	7	11	NULL	NULL	NULL	NORE	GP		is					N-Oct-3 responsive element	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_5_1513_s_35	15767276	A detailed compilation of the available POU/DNA complex structures, as well as a combination of molecular modeling, DNA footprinting and electrophoretic mobility shift assay (EMSA) have enabled us to (i) uncover a new mode of homodimerization adopted by the N-Oct-3 POU domain bound to the respective neuronal AADC and CRH gene promoters, (ii) demonstrate that this pattern is induced by a novel structural motif, the NORE (N-Oct-3 responsive element) and (iii) understand how the same structural motif can also induce the formation of a heterodimer in association with HNF-3beta DBD.	bind
42182	6	9947	7	11	NULL	NULL	NULL	statement 3	GP		is induced by									NORE	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_5_1513_s_35	15767276	A detailed compilation of the available POU/DNA complex structures, as well as a combination of molecular modeling, DNA footprinting and electrophoretic mobility shift assay (EMSA) have enabled us to (i) uncover a new mode of homodimerization adopted by the N-Oct-3 POU domain bound to the respective neuronal AADC and CRH gene promoters, (ii) demonstrate that this pattern is induced by a novel structural motif, the NORE (N-Oct-3 responsive element) and (iii) understand how the same structural motif can also induce the formation of a heterodimer in association with HNF-3beta DBD.	bind
42183	7	9947	7	11	NULL	NULL	NULL	N-Oct-3	GP		heterodimerizes with			POU domain		HNF-3beta	GP		DBD		NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_5_1513_s_35	15767276	A detailed compilation of the available POU/DNA complex structures, as well as a combination of molecular modeling, DNA footprinting and electrophoretic mobility shift assay (EMSA) have enabled us to (i) uncover a new mode of homodimerization adopted by the N-Oct-3 POU domain bound to the respective neuronal AADC and CRH gene promoters, (ii) demonstrate that this pattern is induced by a novel structural motif, the NORE (N-Oct-3 responsive element) and (iii) understand how the same structural motif can also induce the formation of a heterodimer in association with HNF-3beta DBD.	bind
42184	8	9947	7	11	NULL	NULL	NULL	NORE	GP		induce					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_5_1513_s_35	15767276	A detailed compilation of the available POU/DNA complex structures, as well as a combination of molecular modeling, DNA footprinting and electrophoretic mobility shift assay (EMSA) have enabled us to (i) uncover a new mode of homodimerization adopted by the N-Oct-3 POU domain bound to the respective neuronal AADC and CRH gene promoters, (ii) demonstrate that this pattern is induced by a novel structural motif, the NORE (N-Oct-3 responsive element) and (iii) understand how the same structural motif can also induce the formation of a heterodimer in association with HNF-3beta DBD.	bind
49021	9	9947	7	11	NULL	NULL	NULL	statement 4	GP		is induced by									NORE	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_5_1513_s_35	15767276	A detailed compilation of the available POU/DNA complex structures, as well as a combination of molecular modeling, DNA footprinting and electrophoretic mobility shift assay (EMSA) have enabled us to (i) uncover a new mode of homodimerization adopted by the N-Oct-3 POU domain bound to the respective neuronal AADC and CRH gene promoters, (ii) demonstrate that this pattern is induced by a novel structural motif, the NORE (N-Oct-3 responsive element) and (iii) understand how the same structural motif can also induce the formation of a heterodimer in association with HNF-3beta DBD.	bind
34956	1	9948	6	11	NULL	NULL	NULL	v-Ha-Ras 	GP		exists as					isomeric conformers	GP	population of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_30363_s_437	10887184	A detailed kinetic analysis of the v-Ha-Ras-RBD interaction is presented in a separate paper,2 where we show v-Ha-Ras exists as a population of isomeric conformers and that A85K-RBD binds a greater proportion of these conformers than wt-RBD, giving rise to the difference in Ras saturation levels.	bind
34957	2	9948	6	11	NULL	NULL	NULL			wt	bind			RBD		statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_30363_s_437	10887184	A detailed kinetic analysis of the v-Ha-Ras-RBD interaction is presented in a separate paper,2 where we show v-Ha-Ras exists as a population of isomeric conformers and that A85K-RBD binds a greater proportion of these conformers than wt-RBD, giving rise to the difference in Ras saturation levels.	bind
34958	3	9948	6	11	NULL	NULL	NULL				bind			A85K-RBD		statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_30363_s_437	10887184	A detailed kinetic analysis of the v-Ha-Ras-RBD interaction is presented in a separate paper,2 where we show v-Ha-Ras exists as a population of isomeric conformers and that A85K-RBD binds a greater proportion of these conformers than wt-RBD, giving rise to the difference in Ras saturation levels.	bind
34959	4	9948	6	11	NULL	NULL	NULL	statement 3	Process	affinity of	is more than					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_30363_s_437	10887184	A detailed kinetic analysis of the v-Ha-Ras-RBD interaction is presented in a separate paper,2 where we show v-Ha-Ras exists as a population of isomeric conformers and that A85K-RBD binds a greater proportion of these conformers than wt-RBD, giving rise to the difference in Ras saturation levels.	bind
34960	5	9948	6	11	NULL	NULL	NULL	statement 4	Process		leads to					Ras	GP	difference in;;saturation levels of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_30363_s_437	10887184	A detailed kinetic analysis of the v-Ha-Ras-RBD interaction is presented in a separate paper,2 where we show v-Ha-Ras exists as a population of isomeric conformers and that A85K-RBD binds a greater proportion of these conformers than wt-RBD, giving rise to the difference in Ras saturation levels.	bind
42305	2	9948	7	11	NULL	NULL	NULL				bind			A85K-RBD 		statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_30363_s_437	10887184	A detailed kinetic analysis of the v-Ha-Ras-RBD interaction is presented in a separate paper,2 where we show v-Ha-Ras exists as a population of isomeric conformers and that A85K-RBD binds a greater proportion of these conformers than wt-RBD, giving rise to the difference in Ras saturation levels.	bind
42306	3	9948	7	11	NULL	NULL	NULL			wt	bind			RBD		statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_30363_s_437	10887184	A detailed kinetic analysis of the v-Ha-Ras-RBD interaction is presented in a separate paper,2 where we show v-Ha-Ras exists as a population of isomeric conformers and that A85K-RBD binds a greater proportion of these conformers than wt-RBD, giving rise to the difference in Ras saturation levels.	bind
42307	4	9948	7	11	NULL	NULL	NULL	statement 1	Process	affinity of	is greater than					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_30363_s_437	10887184	A detailed kinetic analysis of the v-Ha-Ras-RBD interaction is presented in a separate paper,2 where we show v-Ha-Ras exists as a population of isomeric conformers and that A85K-RBD binds a greater proportion of these conformers than wt-RBD, giving rise to the difference in Ras saturation levels.	bind
49022	1	9948	7	11	NULL	NULL	NULL	v-Ha-Ras	GP		exists as					isomeric conformers	GP	population of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_30363_s_437	10887184	A detailed kinetic analysis of the v-Ha-Ras-RBD interaction is presented in a separate paper,2 where we show v-Ha-Ras exists as a population of isomeric conformers and that A85K-RBD binds a greater proportion of these conformers than wt-RBD, giving rise to the difference in Ras saturation levels.	bind
49023	5	9948	7	11	NULL	NULL	NULL	statement 4	Process		leads to					Ras	GP	difference in;;saturation levels of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_30363_s_437	10887184	A detailed kinetic analysis of the v-Ha-Ras-RBD interaction is presented in a separate paper,2 where we show v-Ha-Ras exists as a population of isomeric conformers and that A85K-RBD binds a greater proportion of these conformers than wt-RBD, giving rise to the difference in Ras saturation levels.	bind
34760	1	9949	6	11	NULL	NULL	NULL	nitrite	Chemical		bind					(P8+)FeIII(H2O)2	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_inorg-chem_45_16_16878967_s_7	16878967	A detailed kinetic studied revealed that nitrite binds to (P8+)FeIII(H2O)2  according to a dissociative mechanism, whereas nitrite binding to (P8+)FeIII(OH)(H2O)  at higher pH follows an associative mechanism, similar to that reported  for the binding of NO to these complexes.	bind
34761	2	9949	6	11	NULL	NULL	NULL	statement 1	Process		follows					dissociative mechanism	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_inorg-chem_45_16_16878967_s_7	16878967	A detailed kinetic studied revealed that nitrite binds to (P8+)FeIII(H2O)2  according to a dissociative mechanism, whereas nitrite binding to (P8+)FeIII(OH)(H2O)  at higher pH follows an associative mechanism, similar to that reported  for the binding of NO to these complexes.	bind
34762	3	9949	6	11	NULL	NULL	NULL	nitrite	Chemical		bind					(P8+)FeIII(OH)(H2O)	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_inorg-chem_45_16_16878967_s_7	16878967	A detailed kinetic studied revealed that nitrite binds to (P8+)FeIII(H2O)2  according to a dissociative mechanism, whereas nitrite binding to (P8+)FeIII(OH)(H2O)  at higher pH follows an associative mechanism, similar to that reported  for the binding of NO to these complexes.	bind
34763	4	9949	6	11	NULL	NULL	NULL	statement 3	Process		follows					associative mechanism	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_inorg-chem_45_16_16878967_s_7	16878967	A detailed kinetic studied revealed that nitrite binds to (P8+)FeIII(H2O)2  according to a dissociative mechanism, whereas nitrite binding to (P8+)FeIII(OH)(H2O)  at higher pH follows an associative mechanism, similar to that reported  for the binding of NO to these complexes.	bind
49024	5	9949	6	11	NULL	NULL	NULL	statement 3	Process		occurs at					pH	QuantityOrMeasure	higher			NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_inorg-chem_45_16_16878967_s_7	16878967	A detailed kinetic studied revealed that nitrite binds to (P8+)FeIII(H2O)2  according to a dissociative mechanism, whereas nitrite binding to (P8+)FeIII(OH)(H2O)  at higher pH follows an associative mechanism, similar to that reported  for the binding of NO to these complexes.	bind
49025	6	9949	6	11	NULL	NULL	NULL	NO	Chemical		bind					(P8+)FeIII(H2O)2	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_inorg-chem_45_16_16878967_s_7	16878967	A detailed kinetic studied revealed that nitrite binds to (P8+)FeIII(H2O)2  according to a dissociative mechanism, whereas nitrite binding to (P8+)FeIII(OH)(H2O)  at higher pH follows an associative mechanism, similar to that reported  for the binding of NO to these complexes.	bind
49026	7	9949	6	11	NULL	NULL	NULL	NO	Chemical		bind					(P8+)FeIII(OH)(H2O)	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_inorg-chem_45_16_16878967_s_7	16878967	A detailed kinetic studied revealed that nitrite binds to (P8+)FeIII(H2O)2  according to a dissociative mechanism, whereas nitrite binding to (P8+)FeIII(OH)(H2O)  at higher pH follows an associative mechanism, similar to that reported  for the binding of NO to these complexes.	bind
49027	8	9949	6	11	NULL	NULL	NULL	statement 1	Process		is similar to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_inorg-chem_45_16_16878967_s_7	16878967	A detailed kinetic studied revealed that nitrite binds to (P8+)FeIII(H2O)2  according to a dissociative mechanism, whereas nitrite binding to (P8+)FeIII(OH)(H2O)  at higher pH follows an associative mechanism, similar to that reported  for the binding of NO to these complexes.	bind
49028	9	9949	6	11	NULL	NULL	NULL	statement 3	Process		is similar to					statement 7	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_inorg-chem_45_16_16878967_s_7	16878967	A detailed kinetic studied revealed that nitrite binds to (P8+)FeIII(H2O)2  according to a dissociative mechanism, whereas nitrite binding to (P8+)FeIII(OH)(H2O)  at higher pH follows an associative mechanism, similar to that reported  for the binding of NO to these complexes.	bind
42185	1	9949	7	11	NULL	NULL	NULL	nitrite	Chemical		binds to					(P8+)FeIII(H2O)2	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_inorg-chem_45_16_16878967_s_7	16878967	A detailed kinetic studied revealed that nitrite binds to (P8+)FeIII(H2O)2  according to a dissociative mechanism, whereas nitrite binding to (P8+)FeIII(OH)(H2O)  at higher pH follows an associative mechanism, similar to that reported  for the binding of NO to these complexes.	bind
42186	2	9949	7	11	NULL	NULL	NULL	statement 1	Process		follows					dissociative mechanism	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_inorg-chem_45_16_16878967_s_7	16878967	A detailed kinetic studied revealed that nitrite binds to (P8+)FeIII(H2O)2  according to a dissociative mechanism, whereas nitrite binding to (P8+)FeIII(OH)(H2O)  at higher pH follows an associative mechanism, similar to that reported  for the binding of NO to these complexes.	bind
42187	3	9949	7	11	NULL	NULL	NULL	nitrite	Chemical		binds to					(P8+)FeIII(OH)(H2O)	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_inorg-chem_45_16_16878967_s_7	16878967	A detailed kinetic studied revealed that nitrite binds to (P8+)FeIII(H2O)2  according to a dissociative mechanism, whereas nitrite binding to (P8+)FeIII(OH)(H2O)  at higher pH follows an associative mechanism, similar to that reported  for the binding of NO to these complexes.	bind
42188	4	9949	7	11	NULL	NULL	NULL	statement 3	Process		occurs at					pH	QuantityOrMeasure	higher			NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_inorg-chem_45_16_16878967_s_7	16878967	A detailed kinetic studied revealed that nitrite binds to (P8+)FeIII(H2O)2  according to a dissociative mechanism, whereas nitrite binding to (P8+)FeIII(OH)(H2O)  at higher pH follows an associative mechanism, similar to that reported  for the binding of NO to these complexes.	bind
42189	5	9949	7	11	NULL	NULL	NULL	statement 3	Process		follows					associative mechanism	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_inorg-chem_45_16_16878967_s_7	16878967	A detailed kinetic studied revealed that nitrite binds to (P8+)FeIII(H2O)2  according to a dissociative mechanism, whereas nitrite binding to (P8+)FeIII(OH)(H2O)  at higher pH follows an associative mechanism, similar to that reported  for the binding of NO to these complexes.	bind
42190	6	9949	7	11	NULL	NULL	NULL	NO	Chemical		bind					 (P8+)FeIII(H2O)2	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_inorg-chem_45_16_16878967_s_7	16878967	A detailed kinetic studied revealed that nitrite binds to (P8+)FeIII(H2O)2  according to a dissociative mechanism, whereas nitrite binding to (P8+)FeIII(OH)(H2O)  at higher pH follows an associative mechanism, similar to that reported  for the binding of NO to these complexes.	bind
42191	7	9949	7	11	NULL	NULL	NULL	NO	Chemical		bind					(P8+)FeIII(OH)(H2O)	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_inorg-chem_45_16_16878967_s_7	16878967	A detailed kinetic studied revealed that nitrite binds to (P8+)FeIII(H2O)2  according to a dissociative mechanism, whereas nitrite binding to (P8+)FeIII(OH)(H2O)  at higher pH follows an associative mechanism, similar to that reported  for the binding of NO to these complexes.	bind
42192	8	9949	7	11	NULL	NULL	NULL	statement 1	Process		is similar to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_inorg-chem_45_16_16878967_s_7	16878967	A detailed kinetic studied revealed that nitrite binds to (P8+)FeIII(H2O)2  according to a dissociative mechanism, whereas nitrite binding to (P8+)FeIII(OH)(H2O)  at higher pH follows an associative mechanism, similar to that reported  for the binding of NO to these complexes.	bind
42193	9	9949	7	11	NULL	NULL	NULL	statement 3	Process		is similar to					statement 7	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_inorg-chem_45_16_16878967_s_7	16878967	A detailed kinetic studied revealed that nitrite binds to (P8+)FeIII(H2O)2  according to a dissociative mechanism, whereas nitrite binding to (P8+)FeIII(OH)(H2O)  at higher pH follows an associative mechanism, similar to that reported  for the binding of NO to these complexes.	bind
35086	1	9951	6	11	NULL	NULL	NULL	N-moesin	GP		is a type of					ERM protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
35087	2	9951	6	11	NULL	NULL	NULL	N-ezrin	GP		is a type of					ERM protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
35088	3	9951	6	11	NULL	NULL	NULL				bind			aa 487-503		N-moesin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
35089	4	9951	6	11	NULL	NULL	NULL				bind			aa 487-503		N-ezrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
35435	5	9951	6	11	NULL	NULL	NULL	N-moesin	GP		bind								S487A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
35437	6	9951	6	11	NULL	NULL	NULL	statement 5	Process	affinity of	is less than					statement 3	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
35438	7	9951	6	11	NULL	NULL	NULL	N-moesin	GP		bind								S489A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
35440	8	9951	6	11	NULL	NULL	NULL	statement 7	Process	affinity of	is less than					statement 3	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
35441	9	9951	6	11	NULL	NULL	NULL	N-moesin	GP		bind								S496A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
35442	10	9951	6	11	NULL	NULL	NULL	statement 9	Process	affinity of	is less than					statement 3	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
35444	11	9951	6	11	NULL	NULL	NULL	N-moesin	GP		bind								T497A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
35445	12	9951	6	11	NULL	NULL	NULL	statement 11	Process	affinity of	is less than					statement 3	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
35447	13	9951	6	11	NULL	NULL	NULL	N-ezrin	GP		bind								S487A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
35448	14	9951	6	11	NULL	NULL	NULL	statement 13	Process	affinity of	is less than					statement 4	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
35449	15	9951	6	11	NULL	NULL	NULL	N-ezrin	GP		bind								S489A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
35451	16	9951	6	11	NULL	NULL	NULL	statement 15	Process	affinity of	is less than					statement 4	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
35453	17	9951	6	11	NULL	NULL	NULL	N-ezrin	GP		bind								S496A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
35454	18	9951	6	11	NULL	NULL	NULL	statement 17	Process	affinity of	is less than					statement 4	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
35455	19	9951	6	11	NULL	NULL	NULL	N-ezrin	GP		bind								T497A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
35456	20	9951	6	11	NULL	NULL	NULL	statement 19	Process	affinity of	is less than					statement 4	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
35457	21	9951	6	11	NULL	NULL	NULL	N-ezrin	GP		bind								R493A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
35458	22	9951	6	11	NULL	NULL	NULL	N-moesin	GP		bind								R493A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
35459	23	9951	6	11	NULL	NULL	NULL	N-ezrin	GP		bind								S503A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
35461	24	9951	6	11	NULL	NULL	NULL	N-moesin	GP		bind								S503A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
42311	1	9951	7	11	NULL	NULL	NULL				bind			aa 487-503 		N-moesin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
42312	2	9951	7	11	NULL	NULL	NULL				bind			aa 487-503 		N-ezrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
42313	3	9951	7	11	NULL	NULL	NULL	N-moesin	GP		bind							point mutant	S487A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
42314	4	9951	7	11	NULL	NULL	NULL	N-moesin	GP		bind							point mutant	S489A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
42315	5	9951	7	11	NULL	NULL	NULL	N-moesin	GP		bind							point mutant	 S496A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
42316	6	9951	7	11	NULL	NULL	NULL	N-moesin	GP		bind							point mutant	T497A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
42317	7	9951	7	11	NULL	NULL	NULL	N-ezrin	GP		bind							point mutant	S487A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
42318	8	9951	7	11	NULL	NULL	NULL	N-ezrin	GP		bind							point mutant	S489A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
42319	9	9951	7	11	NULL	NULL	NULL	N-ezrin	GP		bind							point mutant	S496A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
42320	10	9951	7	11	NULL	NULL	NULL	N-ezrin	GP		bind							point mutant	T497A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
42321	11	9951	7	11	NULL	NULL	NULL	N-ezrin	GP		bind							point mutant	R493A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
42322	12	9951	7	11	NULL	NULL	NULL	N-ezrin	GP		bind							point mutant	S503A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
57602	13	9951	7	11	NULL	NULL	NULL	N-moesin	GP		bind							point mutant	R493A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
57603	14	9951	7	11	NULL	NULL	NULL	N-moesin	GP		bind							point mutant	S503A		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
57604	15	9951	7	11	NULL	NULL	NULL	statement 3	Process	affinity of	is lesser than					statement 1	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
57605	16	9951	7	11	NULL	NULL	NULL	statement 4	Process	affinity of	is lesser than					statement 1	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
57606	17	9951	7	11	NULL	NULL	NULL	statement 5	Process	affinity of	is lesser than					statement 1	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
57607	18	9951	7	11	NULL	NULL	NULL	statement 6	Process	affinity of	is lesser than					statement 1	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
57608	19	9951	7	11	NULL	NULL	NULL	statement 7	Process	affinity of	is lesser than					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
57609	20	9951	7	11	NULL	NULL	NULL	statement 8	Process	affinity of	is lesser than					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
57610	21	9951	7	11	NULL	NULL	NULL	statement 9	Process	affinity of	is lesser than					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
57611	22	9951	7	11	NULL	NULL	NULL	statement 10	Process	affinity of	is lesser than					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
57612	23	9951	7	11	NULL	NULL	NULL	N-moesin	GP		is a type of					ERM protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
57613	24	9951	7	11	NULL	NULL	NULL	N-ezrin	GP		is a type of					ERM protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10400_s_229	11784723	A detailed mutational analysis of this region (residues 487-503) showed that binding of N-moesin and N-ezrin to S487A, S489A, S496A, and T497A point mutations was reduced, whereas R493A and S503A mutants bound both ERM proteins at levels comparable with those of the wild type protein (Fig.  7,  A-C).	bind
34772	1	9952	6	11	NULL	NULL	NULL	Sir2 proteins	GP		mediates					nicotinamide	Chemical	clevage of 			NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_23_8563_s_14	15150415	A detailed structural understanding of how the Sir2 proteins mediate nicotinamide cleavage and ADP-ribose transfer to acetate has been hampered by the difficulty in trapping a Sir2 protein bound to a form of NAD+ containing an ordered nicotinamide group ( ,  ,  ,  ).	bind
49030	2	9952	6	11	NULL	NULL	NULL	ADP-ribose	Chemical		is transfered to					acetate	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_23_8563_s_14	15150415	A detailed structural understanding of how the Sir2 proteins mediate nicotinamide cleavage and ADP-ribose transfer to acetate has been hampered by the difficulty in trapping a Sir2 protein bound to a form of NAD+ containing an ordered nicotinamide group ( ,  ,  ,  ).	bind
49031	3	9952	6	11	NULL	NULL	NULL	Sir2 proteins	GP		mediate					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_23_8563_s_14	15150415	A detailed structural understanding of how the Sir2 proteins mediate nicotinamide cleavage and ADP-ribose transfer to acetate has been hampered by the difficulty in trapping a Sir2 protein bound to a form of NAD+ containing an ordered nicotinamide group ( ,  ,  ,  ).	bind
49032	4	9952	6	11	NULL	NULL	NULL	NAD+	Chemical		contains					nicotinamide group	Chemical	ordered			NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_23_8563_s_14	15150415	A detailed structural understanding of how the Sir2 proteins mediate nicotinamide cleavage and ADP-ribose transfer to acetate has been hampered by the difficulty in trapping a Sir2 protein bound to a form of NAD+ containing an ordered nicotinamide group ( ,  ,  ,  ).	bind
49033	5	9952	6	11	NULL	NULL	NULL	Sir2 protein	GP		bind					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_23_8563_s_14	15150415	A detailed structural understanding of how the Sir2 proteins mediate nicotinamide cleavage and ADP-ribose transfer to acetate has been hampered by the difficulty in trapping a Sir2 protein bound to a form of NAD+ containing an ordered nicotinamide group ( ,  ,  ,  ).	bind
42323	1	9952	7	11	NULL	NULL	NULL	 Sir2 proteins	GP		mediate					nicotinamide	Chemical	cleavage of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_23_8563_s_14	15150415	A detailed structural understanding of how the Sir2 proteins mediate nicotinamide cleavage and ADP-ribose transfer to acetate has been hampered by the difficulty in trapping a Sir2 protein bound to a form of NAD+ containing an ordered nicotinamide group ( ,  ,  ,  ).	bind
42324	2	9952	7	11	NULL	NULL	NULL	 ADP-ribose	Chemical		is transfered to					acetate	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_23_8563_s_14	15150415	A detailed structural understanding of how the Sir2 proteins mediate nicotinamide cleavage and ADP-ribose transfer to acetate has been hampered by the difficulty in trapping a Sir2 protein bound to a form of NAD+ containing an ordered nicotinamide group ( ,  ,  ,  ).	bind
42325	3	9952	7	11	NULL	NULL	NULL	Sir2 proteins	GP		mediate					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_23_8563_s_14	15150415	A detailed structural understanding of how the Sir2 proteins mediate nicotinamide cleavage and ADP-ribose transfer to acetate has been hampered by the difficulty in trapping a Sir2 protein bound to a form of NAD+ containing an ordered nicotinamide group ( ,  ,  ,  ).	bind
42326	5	9952	7	11	NULL	NULL	NULL	Sir2 protein	GP		bind					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_23_8563_s_14	15150415	A detailed structural understanding of how the Sir2 proteins mediate nicotinamide cleavage and ADP-ribose transfer to acetate has been hampered by the difficulty in trapping a Sir2 protein bound to a form of NAD+ containing an ordered nicotinamide group ( ,  ,  ,  ).	bind
49029	4	9952	7	11	NULL	NULL	NULL	NAD+	Chemical		contains					nicotinamide group	Chemical	ordered			NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_23_8563_s_14	15150415	A detailed structural understanding of how the Sir2 proteins mediate nicotinamide cleavage and ADP-ribose transfer to acetate has been hampered by the difficulty in trapping a Sir2 protein bound to a form of NAD+ containing an ordered nicotinamide group ( ,  ,  ,  ).	bind
34773	1	9953	6	11	NULL	NULL	NULL	Cak1p	GP		bind					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_9_2545_s_366	9725911	A detailed study of the ATP-binding properties of Cak1p will be published elsewhere (Enke, Holmes, Kaldis, and Solomon).	bind
42327	1	9953	7	11	NULL	NULL	NULL	Cak1p	GP		bind					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_9_2545_s_366	9725911	A detailed study of the ATP-binding properties of Cak1p will be published elsewhere (Enke, Holmes, Kaldis, and Solomon).	bind
35090	1	9954	6	11	NULL	NULL	NULL	GM	GP		bind					Hsp90	GP		N-terminal ADP/ATP binding site		NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_3_289_s_51	11306353	A detailed study of the mode of binding of GM (Protein Data Bank code 1YET), RD (code 1BGQ) and ADP (code 1AMW) to the Hsp90 N-terminal ADP/ATP binding site revealed several important factors to be considered in designing a molecule that would interact with this pocket: (1) a key interaction between the inhibitor and the Asp93/Ser52 at the base of the pocket, (2) interactions at the top involving Lys112, Lys58 and hydrogen acceptor functionalities on the inhibitor, (3) a hydrophobic pocket that lies midway in the binding site and that is constituted by Met98, Val150, Leu107, Leu103, Phe138 and Val186 (the amino acid numbering as in human Hsp90  ).	bind
35091	2	9954	6	11	NULL	NULL	NULL	RD	GP		bind					Hsp90	GP		N-terminal ADP/ATP binding site		NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_3_289_s_51	11306353	A detailed study of the mode of binding of GM (Protein Data Bank code 1YET), RD (code 1BGQ) and ADP (code 1AMW) to the Hsp90 N-terminal ADP/ATP binding site revealed several important factors to be considered in designing a molecule that would interact with this pocket: (1) a key interaction between the inhibitor and the Asp93/Ser52 at the base of the pocket, (2) interactions at the top involving Lys112, Lys58 and hydrogen acceptor functionalities on the inhibitor, (3) a hydrophobic pocket that lies midway in the binding site and that is constituted by Met98, Val150, Leu107, Leu103, Phe138 and Val186 (the amino acid numbering as in human Hsp90  ).	bind
35092	3	9954	6	11	NULL	NULL	NULL	ADP	Chemical		bind					Hsp90	GP		N-terminal ADP/ATP binding site		NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_3_289_s_51	11306353	A detailed study of the mode of binding of GM (Protein Data Bank code 1YET), RD (code 1BGQ) and ADP (code 1AMW) to the Hsp90 N-terminal ADP/ATP binding site revealed several important factors to be considered in designing a molecule that would interact with this pocket: (1) a key interaction between the inhibitor and the Asp93/Ser52 at the base of the pocket, (2) interactions at the top involving Lys112, Lys58 and hydrogen acceptor functionalities on the inhibitor, (3) a hydrophobic pocket that lies midway in the binding site and that is constituted by Met98, Val150, Leu107, Leu103, Phe138 and Val186 (the amino acid numbering as in human Hsp90  ).	bind
35466	4	9954	6	11	NULL	NULL	NULL	Hsp90	GP	human	constitute			Met98;; Val150;; Leu107;; Leu103;; Phe138;; Val186		HSP90	GP		hydrophobic pocket in N-terminal ADP/ATP binding site		NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_3_289_s_51	11306353	A detailed study of the mode of binding of GM (Protein Data Bank code 1YET), RD (code 1BGQ) and ADP (code 1AMW) to the Hsp90 N-terminal ADP/ATP binding site revealed several important factors to be considered in designing a molecule that would interact with this pocket: (1) a key interaction between the inhibitor and the Asp93/Ser52 at the base of the pocket, (2) interactions at the top involving Lys112, Lys58 and hydrogen acceptor functionalities on the inhibitor, (3) a hydrophobic pocket that lies midway in the binding site and that is constituted by Met98, Val150, Leu107, Leu103, Phe138 and Val186 (the amino acid numbering as in human Hsp90  ).	bind
42328	1	9954	7	11	NULL	NULL	NULL	GM	GP		bind					 Hsp90	GP		N-terminal ADP/ATP binding site		NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_3_289_s_51	11306353	A detailed study of the mode of binding of GM (Protein Data Bank code 1YET), RD (code 1BGQ) and ADP (code 1AMW) to the Hsp90 N-terminal ADP/ATP binding site revealed several important factors to be considered in designing a molecule that would interact with this pocket: (1) a key interaction between the inhibitor and the Asp93/Ser52 at the base of the pocket, (2) interactions at the top involving Lys112, Lys58 and hydrogen acceptor functionalities on the inhibitor, (3) a hydrophobic pocket that lies midway in the binding site and that is constituted by Met98, Val150, Leu107, Leu103, Phe138 and Val186 (the amino acid numbering as in human Hsp90  ).	bind
42329	2	9954	7	11	NULL	NULL	NULL	RD	GP		bind					Hsp90	GP		N-terminal ADP/ATP binding site		NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_3_289_s_51	11306353	A detailed study of the mode of binding of GM (Protein Data Bank code 1YET), RD (code 1BGQ) and ADP (code 1AMW) to the Hsp90 N-terminal ADP/ATP binding site revealed several important factors to be considered in designing a molecule that would interact with this pocket: (1) a key interaction between the inhibitor and the Asp93/Ser52 at the base of the pocket, (2) interactions at the top involving Lys112, Lys58 and hydrogen acceptor functionalities on the inhibitor, (3) a hydrophobic pocket that lies midway in the binding site and that is constituted by Met98, Val150, Leu107, Leu103, Phe138 and Val186 (the amino acid numbering as in human Hsp90  ).	bind
42330	3	9954	7	11	NULL	NULL	NULL	ADP	Chemical		bind					Hsp90	GP		N-terminal ADP/ATP binding site		NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_3_289_s_51	11306353	A detailed study of the mode of binding of GM (Protein Data Bank code 1YET), RD (code 1BGQ) and ADP (code 1AMW) to the Hsp90 N-terminal ADP/ATP binding site revealed several important factors to be considered in designing a molecule that would interact with this pocket: (1) a key interaction between the inhibitor and the Asp93/Ser52 at the base of the pocket, (2) interactions at the top involving Lys112, Lys58 and hydrogen acceptor functionalities on the inhibitor, (3) a hydrophobic pocket that lies midway in the binding site and that is constituted by Met98, Val150, Leu107, Leu103, Phe138 and Val186 (the amino acid numbering as in human Hsp90  ).	bind
42344	4	9954	7	11	NULL	NULL	NULL	Hsp90	GP	human	constitute			Met98;;Val150;;Leu107;;Leu103;;Phe138;;Val186		Hsp90	GP		hydrophobic pocket in N-terminal ADP/ATPbinding site		NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_3_289_s_51	11306353	A detailed study of the mode of binding of GM (Protein Data Bank code 1YET), RD (code 1BGQ) and ADP (code 1AMW) to the Hsp90 N-terminal ADP/ATP binding site revealed several important factors to be considered in designing a molecule that would interact with this pocket: (1) a key interaction between the inhibitor and the Asp93/Ser52 at the base of the pocket, (2) interactions at the top involving Lys112, Lys58 and hydrogen acceptor functionalities on the inhibitor, (3) a hydrophobic pocket that lies midway in the binding site and that is constituted by Met98, Val150, Leu107, Leu103, Phe138 and Val186 (the amino acid numbering as in human Hsp90  ).	bind
34774	1	9955	6	11	NULL	NULL	NULL	E.coli	Organism	P-fimbriated	bind					uroepithelial cells	Cell	human			NULL		NULL	NULL	NULL	NULL	gw70_microbesinfect_8_3_938_s_47	16460984	A detailed study using a different inhibitor of GlcCer synthase,  N-butyl deoxynojirimycin (an N-butylated amino sugar-like compound), also blockaded  P-fimbriated  E. coli binding to human uroepithelial cells   [15].	bind
34775	2	9955	6	11	NULL	NULL	NULL	N-butyl deoxynojirimycin	Chemical		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_microbesinfect_8_3_938_s_47	16460984	A detailed study using a different inhibitor of GlcCer synthase,  N-butyl deoxynojirimycin (an N-butylated amino sugar-like compound), also blockaded  P-fimbriated  E. coli binding to human uroepithelial cells   [15].	bind
34776	3	9955	6	11	NULL	NULL	NULL	N-butyl deoxynojirimycin	Chemical		is an					N-butylated amino sugar-like compound	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_microbesinfect_8_3_938_s_47	16460984	A detailed study using a different inhibitor of GlcCer synthase,  N-butyl deoxynojirimycin (an N-butylated amino sugar-like compound), also blockaded  P-fimbriated  E. coli binding to human uroepithelial cells   [15].	bind
49034	4	9955	6	11	NULL	NULL	NULL	N-butyl deoxynojirimycin	Chemical		is an inhibitor of					GlcCer synthase	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbesinfect_8_3_938_s_47	16460984	A detailed study using a different inhibitor of GlcCer synthase,  N-butyl deoxynojirimycin (an N-butylated amino sugar-like compound), also blockaded  P-fimbriated  E. coli binding to human uroepithelial cells   [15].	bind
42354	1	9955	7	11	NULL	NULL	NULL	E. coli	Organism	P-fimbriated	bind					uroepithelial cells	Cell	human			NULL		NULL	NULL	NULL	NULL	gw70_microbesinfect_8_3_938_s_47	16460984	A detailed study using a different inhibitor of GlcCer synthase,  N-butyl deoxynojirimycin (an N-butylated amino sugar-like compound), also blockaded  P-fimbriated  E. coli binding to human uroepithelial cells   [15].	bind
42355	2	9955	7	11	NULL	NULL	NULL	N-butyl deoxynojirimycin	Chemical		is an inhibitor of					GlcCer synthase	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbesinfect_8_3_938_s_47	16460984	A detailed study using a different inhibitor of GlcCer synthase,  N-butyl deoxynojirimycin (an N-butylated amino sugar-like compound), also blockaded  P-fimbriated  E. coli binding to human uroepithelial cells   [15].	bind
42356	3	9955	7	11	NULL	NULL	NULL	N-butyl deoxynojirimycin	Chemical		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_microbesinfect_8_3_938_s_47	16460984	A detailed study using a different inhibitor of GlcCer synthase,  N-butyl deoxynojirimycin (an N-butylated amino sugar-like compound), also blockaded  P-fimbriated  E. coli binding to human uroepithelial cells   [15].	bind
42357	4	9955	7	11	NULL	NULL	NULL	N-butyl deoxynojirimycin	Chemical		is					N-butylated amino sugar-like compound	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_microbesinfect_8_3_938_s_47	16460984	A detailed study using a different inhibitor of GlcCer synthase,  N-butyl deoxynojirimycin (an N-butylated amino sugar-like compound), also blockaded  P-fimbriated  E. coli binding to human uroepithelial cells   [15].	bind
34777	1	9956	6	11	NULL	NULL	NULL	PYY	GP	125I-labeled	is an agonist of		potent	3-36		Y2	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_115_4_1035_s_148	12453477	A detailed Y2-binding study of  Schwarzer et al. (1998) demonstrated that [125]PYY 3-36 is a potent Y2 agonist with much less affinities for Y1, Y4 and Y5 receptors, indicating that this ligand may bind mainly to Y2 receptors.	bind
34778	2	9956	6	11	NULL	NULL	NULL	PYY 	GP	125I-labeled	bind		mainly;;may	3-36		Y2 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_115_4_1035_s_148	12453477	A detailed Y2-binding study of  Schwarzer et al. (1998) demonstrated that [125]PYY 3-36 is a potent Y2 agonist with much less affinities for Y1, Y4 and Y5 receptors, indicating that this ligand may bind mainly to Y2 receptors.	bind
34779	3	9956	6	11	NULL	NULL	NULL	PYY	GP	125I-labeled	affinity for		less	3-36		Y1 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_115_4_1035_s_148	12453477	A detailed Y2-binding study of  Schwarzer et al. (1998) demonstrated that [125]PYY 3-36 is a potent Y2 agonist with much less affinities for Y1, Y4 and Y5 receptors, indicating that this ligand may bind mainly to Y2 receptors.	bind
34780	4	9956	6	11	NULL	NULL	NULL	PYY	GP	125I-labeled	affinity for		less	3-36		Y4 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_115_4_1035_s_148	12453477	A detailed Y2-binding study of  Schwarzer et al. (1998) demonstrated that [125]PYY 3-36 is a potent Y2 agonist with much less affinities for Y1, Y4 and Y5 receptors, indicating that this ligand may bind mainly to Y2 receptors.	bind
34781	5	9956	6	11	NULL	NULL	NULL	PYY	GP	125I-labeled	affinity for		less	3-36		Y5 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_115_4_1035_s_148	12453477	A detailed Y2-binding study of  Schwarzer et al. (1998) demonstrated that [125]PYY 3-36 is a potent Y2 agonist with much less affinities for Y1, Y4 and Y5 receptors, indicating that this ligand may bind mainly to Y2 receptors.	bind
42358	1	9956	7	11	NULL	NULL	NULL	PYY	GP	125I-labeled	is an agonist of		potent	3-36		Y2	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_115_4_1035_s_148	12453477	A detailed Y2-binding study of  Schwarzer et al. (1998) demonstrated that [125]PYY 3-36 is a potent Y2 agonist with much less affinities for Y1, Y4 and Y5 receptors, indicating that this ligand may bind mainly to Y2 receptors.	bind
42359	2	9956	7	11	NULL	NULL	NULL	PYY	GP	125I-labeled	affinity for		less	3-36		Y1 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_115_4_1035_s_148	12453477	A detailed Y2-binding study of  Schwarzer et al. (1998) demonstrated that [125]PYY 3-36 is a potent Y2 agonist with much less affinities for Y1, Y4 and Y5 receptors, indicating that this ligand may bind mainly to Y2 receptors.	bind
42360	3	9956	7	11	NULL	NULL	NULL	PYY	GP	125I-labeled	affinity for		less	3-36		Y4 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_115_4_1035_s_148	12453477	A detailed Y2-binding study of  Schwarzer et al. (1998) demonstrated that [125]PYY 3-36 is a potent Y2 agonist with much less affinities for Y1, Y4 and Y5 receptors, indicating that this ligand may bind mainly to Y2 receptors.	bind
42362	4	9956	7	11	NULL	NULL	NULL	PYY	GP	125I-labeled	affinity for		less	3-36		Y5 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_115_4_1035_s_148	12453477	A detailed Y2-binding study of  Schwarzer et al. (1998) demonstrated that [125]PYY 3-36 is a potent Y2 agonist with much less affinities for Y1, Y4 and Y5 receptors, indicating that this ligand may bind mainly to Y2 receptors.	bind
42363	5	9956	7	11	NULL	NULL	NULL	PYY	GP	125I-labeled	bind		mainly;;may	3-36		Y2 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_115_4_1035_s_148	12453477	A detailed Y2-binding study of  Schwarzer et al. (1998) demonstrated that [125]PYY 3-36 is a potent Y2 agonist with much less affinities for Y1, Y4 and Y5 receptors, indicating that this ligand may bind mainly to Y2 receptors.	bind
34782	1	9957	6	11	NULL	NULL	NULL	ARF	GP		bind					GST-NCS-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_7_6047_s_106	15576365	A detectable signal was observed only for ARF1 binding to GST-NCS-1 in the presence  of free Ca2+.	bind
34783	2	9957	6	11	NULL	NULL	NULL	statement 1	Process		in the presence of					Ca2+	Chemical	free			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_7_6047_s_106	15576365	A detectable signal was observed only for ARF1 binding to GST-NCS-1 in the presence  of free Ca2+.	bind
42372	1	9957	7	11	NULL	NULL	NULL	 ARF1	GP		binds					GST-NCS-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_7_6047_s_106	15576365	A detectable signal was observed only for ARF1 binding to GST-NCS-1 in the presence  of free Ca2+.	bind
42373	2	9957	7	11	NULL	NULL	NULL	statement 1	Process		in the presence of					Ca2+	Chemical	free			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_7_6047_s_106	15576365	A detectable signal was observed only for ARF1 binding to GST-NCS-1 in the presence  of free Ca2+.	bind
34784	1	9959	6	11	NULL	NULL	NULL	determinant linked to CLA	GP		bind					E-selectin	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_22_12899_s_25	14566059	A determinant linked to cutaneous lymphocyte-associated antigen (CLA) ( ) binds to E-selectin to assist lymphocyte trafficking to skin.	bind
34785	2	9959	6	11	NULL	NULL	NULL	CLA	GP		is					cutaneous lymphocyte-associated antigen	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_22_12899_s_25	14566059	A determinant linked to cutaneous lymphocyte-associated antigen (CLA) ( ) binds to E-selectin to assist lymphocyte trafficking to skin.	bind
34786	3	9959	6	11	NULL	NULL	NULL	lymphocyte	Cell		is trafficked to					skin	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_22_12899_s_25	14566059	A determinant linked to cutaneous lymphocyte-associated antigen (CLA) ( ) binds to E-selectin to assist lymphocyte trafficking to skin.	bind
49535	4	9959	6	11	NULL	NULL	NULL	statement 1	Process		assist					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_22_12899_s_25	14566059	A determinant linked to cutaneous lymphocyte-associated antigen (CLA) ( ) binds to E-selectin to assist lymphocyte trafficking to skin.	bind
42376	1	9959	7	11	NULL	NULL	NULL	 determinant linked to CLA	GP		binds to					E-selectin	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_22_12899_s_25	14566059	A determinant linked to cutaneous lymphocyte-associated antigen (CLA) ( ) binds to E-selectin to assist lymphocyte trafficking to skin.	bind
42377	2	9959	7	11	NULL	NULL	NULL	lymphocyte	Cell		is trafficked to					skin	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_22_12899_s_25	14566059	A determinant linked to cutaneous lymphocyte-associated antigen (CLA) ( ) binds to E-selectin to assist lymphocyte trafficking to skin.	bind
42378	3	9959	7	11	NULL	NULL	NULL	statement 1	Process		assist					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_22_12899_s_25	14566059	A determinant linked to cutaneous lymphocyte-associated antigen (CLA) ( ) binds to E-selectin to assist lymphocyte trafficking to skin.	bind
42379	4	9959	7	11	NULL	NULL	NULL	CLA	GP		is					cutaneous lymphocyte-associated antigen	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_22_12899_s_25	14566059	A determinant linked to cutaneous lymphocyte-associated antigen (CLA) ( ) binds to E-selectin to assist lymphocyte trafficking to skin.	bind
34962	1	9960	6	11	NULL	NULL	NULL	DGK-zeta	GP	mutant	mimics							phosphorylation of	MARCKS domain		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7289_s_12	16055737	A DGK-zeta mutant that mimics phosphorylation of the MARCKS domain was unable to bind an activated Rac1 mutant (Rac1V12) and phorbol myristate acetate-induced protein kinase C activation inhibited the interaction of DGK-zeta with Rac1V12, suggesting protein kinase C-mediated phosphorylation of the MARCKS domain negatively regulates DGK-zeta binding to active Rac1.	bind
34963	2	9960	6	11	NULL	NULL	NULL	DGK-zeta	GP	mutant	does not bind					Rac1	GP	activated;; mutant			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7289_s_12	16055737	A DGK-zeta mutant that mimics phosphorylation of the MARCKS domain was unable to bind an activated Rac1 mutant (Rac1V12) and phorbol myristate acetate-induced protein kinase C activation inhibited the interaction of DGK-zeta with Rac1V12, suggesting protein kinase C-mediated phosphorylation of the MARCKS domain negatively regulates DGK-zeta binding to active Rac1.	bind
34964	3	9960	6	11	NULL	NULL	NULL	DGK-zeta	GP		interacts with					Rac1V12	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7289_s_12	16055737	A DGK-zeta mutant that mimics phosphorylation of the MARCKS domain was unable to bind an activated Rac1 mutant (Rac1V12) and phorbol myristate acetate-induced protein kinase C activation inhibited the interaction of DGK-zeta with Rac1V12, suggesting protein kinase C-mediated phosphorylation of the MARCKS domain negatively regulates DGK-zeta binding to active Rac1.	bind
34965	4	9960	6	11	NULL	NULL	NULL	protein kinase C	GP	activation of	is induced by					phorbol myristate acetate	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7289_s_12	16055737	A DGK-zeta mutant that mimics phosphorylation of the MARCKS domain was unable to bind an activated Rac1 mutant (Rac1V12) and phorbol myristate acetate-induced protein kinase C activation inhibited the interaction of DGK-zeta with Rac1V12, suggesting protein kinase C-mediated phosphorylation of the MARCKS domain negatively regulates DGK-zeta binding to active Rac1.	bind
34966	5	9960	6	11	NULL	NULL	NULL	statement 4	Process		inhibits					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7289_s_12	16055737	A DGK-zeta mutant that mimics phosphorylation of the MARCKS domain was unable to bind an activated Rac1 mutant (Rac1V12) and phorbol myristate acetate-induced protein kinase C activation inhibited the interaction of DGK-zeta with Rac1V12, suggesting protein kinase C-mediated phosphorylation of the MARCKS domain negatively regulates DGK-zeta binding to active Rac1.	bind
34967	6	9960	6	11	NULL	NULL	NULL			phosphorylation of	is mediated by			MARCKS domain		protein kinase C	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7289_s_12	16055737	A DGK-zeta mutant that mimics phosphorylation of the MARCKS domain was unable to bind an activated Rac1 mutant (Rac1V12) and phorbol myristate acetate-induced protein kinase C activation inhibited the interaction of DGK-zeta with Rac1V12, suggesting protein kinase C-mediated phosphorylation of the MARCKS domain negatively regulates DGK-zeta binding to active Rac1.	bind
34968	7	9960	6	11	NULL	NULL	NULL	DGK-zeta	GP		bind					Rac1	GP	active			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7289_s_12	16055737	A DGK-zeta mutant that mimics phosphorylation of the MARCKS domain was unable to bind an activated Rac1 mutant (Rac1V12) and phorbol myristate acetate-induced protein kinase C activation inhibited the interaction of DGK-zeta with Rac1V12, suggesting protein kinase C-mediated phosphorylation of the MARCKS domain negatively regulates DGK-zeta binding to active Rac1.	bind
34969	8	9960	6	11	NULL	NULL	NULL	statement 6	Process		regulates		negatively			statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7289_s_12	16055737	A DGK-zeta mutant that mimics phosphorylation of the MARCKS domain was unable to bind an activated Rac1 mutant (Rac1V12) and phorbol myristate acetate-induced protein kinase C activation inhibited the interaction of DGK-zeta with Rac1V12, suggesting protein kinase C-mediated phosphorylation of the MARCKS domain negatively regulates DGK-zeta binding to active Rac1.	bind
49035	9	9960	6	11	NULL	NULL	NULL	Rac1V12	GP		is					activated Rac1 mutant	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7289_s_12	16055737	A DGK-zeta mutant that mimics phosphorylation of the MARCKS domain was unable to bind an activated Rac1 mutant (Rac1V12) and phorbol myristate acetate-induced protein kinase C activation inhibited the interaction of DGK-zeta with Rac1V12, suggesting protein kinase C-mediated phosphorylation of the MARCKS domain negatively regulates DGK-zeta binding to active Rac1.	bind
42381	1	9960	7	11	NULL	NULL	NULL	DGK-zeta	GP	mutant	mimics							phosphorylation of	MARCKS domain		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7289_s_12	16055737	A DGK-zeta mutant that mimics phosphorylation of the MARCKS domain was unable to bind an activated Rac1 mutant (Rac1V12) and phorbol myristate acetate-induced protein kinase C activation inhibited the interaction of DGK-zeta with Rac1V12, suggesting protein kinase C-mediated phosphorylation of the MARCKS domain negatively regulates DGK-zeta binding to active Rac1.	bind
42382	2	9960	7	11	NULL	NULL	NULL	statement 1	GP		does not bind					Rac1	GP	activated;;mutant			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7289_s_12	16055737	A DGK-zeta mutant that mimics phosphorylation of the MARCKS domain was unable to bind an activated Rac1 mutant (Rac1V12) and phorbol myristate acetate-induced protein kinase C activation inhibited the interaction of DGK-zeta with Rac1V12, suggesting protein kinase C-mediated phosphorylation of the MARCKS domain negatively regulates DGK-zeta binding to active Rac1.	bind
42383	3	9960	7	11	NULL	NULL	NULL	phorbol myristate acetate	Chemical		induce					protein kinase C 	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7289_s_12	16055737	A DGK-zeta mutant that mimics phosphorylation of the MARCKS domain was unable to bind an activated Rac1 mutant (Rac1V12) and phorbol myristate acetate-induced protein kinase C activation inhibited the interaction of DGK-zeta with Rac1V12, suggesting protein kinase C-mediated phosphorylation of the MARCKS domain negatively regulates DGK-zeta binding to active Rac1.	bind
42384	4	9960	7	11	NULL	NULL	NULL	DGK-zeta	GP		interacts with					Rac1V12	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7289_s_12	16055737	A DGK-zeta mutant that mimics phosphorylation of the MARCKS domain was unable to bind an activated Rac1 mutant (Rac1V12) and phorbol myristate acetate-induced protein kinase C activation inhibited the interaction of DGK-zeta with Rac1V12, suggesting protein kinase C-mediated phosphorylation of the MARCKS domain negatively regulates DGK-zeta binding to active Rac1.	bind
42385	5	9960	7	11	NULL	NULL	NULL	statement 3	Process		inhibits					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7289_s_12	16055737	A DGK-zeta mutant that mimics phosphorylation of the MARCKS domain was unable to bind an activated Rac1 mutant (Rac1V12) and phorbol myristate acetate-induced protein kinase C activation inhibited the interaction of DGK-zeta with Rac1V12, suggesting protein kinase C-mediated phosphorylation of the MARCKS domain negatively regulates DGK-zeta binding to active Rac1.	bind
42386	6	9960	7	11	NULL	NULL	NULL	 protein kinase C	GP		mediates							phosphorylation of	MARCKS domain		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7289_s_12	16055737	A DGK-zeta mutant that mimics phosphorylation of the MARCKS domain was unable to bind an activated Rac1 mutant (Rac1V12) and phorbol myristate acetate-induced protein kinase C activation inhibited the interaction of DGK-zeta with Rac1V12, suggesting protein kinase C-mediated phosphorylation of the MARCKS domain negatively regulates DGK-zeta binding to active Rac1.	bind
42387	7	9960	7	11	NULL	NULL	NULL	DGK-zeta	GP		bind					Rac1	GP	active			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7289_s_12	16055737	A DGK-zeta mutant that mimics phosphorylation of the MARCKS domain was unable to bind an activated Rac1 mutant (Rac1V12) and phorbol myristate acetate-induced protein kinase C activation inhibited the interaction of DGK-zeta with Rac1V12, suggesting protein kinase C-mediated phosphorylation of the MARCKS domain negatively regulates DGK-zeta binding to active Rac1.	bind
42388	8	9960	7	11	NULL	NULL	NULL	statement 6	Process		regulates		negatively			statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7289_s_12	16055737	A DGK-zeta mutant that mimics phosphorylation of the MARCKS domain was unable to bind an activated Rac1 mutant (Rac1V12) and phorbol myristate acetate-induced protein kinase C activation inhibited the interaction of DGK-zeta with Rac1V12, suggesting protein kinase C-mediated phosphorylation of the MARCKS domain negatively regulates DGK-zeta binding to active Rac1.	bind
42389	9	9960	7	11	NULL	NULL	NULL	statement 5	Process		suggests					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7289_s_12	16055737	A DGK-zeta mutant that mimics phosphorylation of the MARCKS domain was unable to bind an activated Rac1 mutant (Rac1V12) and phorbol myristate acetate-induced protein kinase C activation inhibited the interaction of DGK-zeta with Rac1V12, suggesting protein kinase C-mediated phosphorylation of the MARCKS domain negatively regulates DGK-zeta binding to active Rac1.	bind
42390	10	9960	7	11	NULL	NULL	NULL	Rac1V12	GP		is					activated Rac1 mutant	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7289_s_12	16055737	A DGK-zeta mutant that mimics phosphorylation of the MARCKS domain was unable to bind an activated Rac1 mutant (Rac1V12) and phorbol myristate acetate-induced protein kinase C activation inhibited the interaction of DGK-zeta with Rac1V12, suggesting protein kinase C-mediated phosphorylation of the MARCKS domain negatively regulates DGK-zeta binding to active Rac1.	bind
34970	1	9961	6	11	NULL	NULL	NULL	C-Raf1	GP		bind					Nef	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_25_15727_s_111	9624170	A Di-aspartic Acid Motif Is Critical for C-Raf1 Binding to Nef-- Since the carboxyl-terminal end of the Nef sequence deleted from the GST-delta41Nef fusion protein above, Leu-His-Pro-Val-Ser-Leu-His-Gly-Met-Asp-Asp-Pro-Glu (amino acids 165-177), also contains the highly conserved pair of aspartic acid residues (positions 174 and 175), we investigated the contributions of this pair of acidic residues to binding of the c-Raf1 protein  in vitro.	bind
34971	2	9961	6	11	NULL	NULL	NULL				is critical for			Di-aspartic Acid Motif 		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_25_15727_s_111	9624170	A Di-aspartic Acid Motif Is Critical for C-Raf1 Binding to Nef-- Since the carboxyl-terminal end of the Nef sequence deleted from the GST-delta41Nef fusion protein above, Leu-His-Pro-Val-Ser-Leu-His-Gly-Met-Asp-Asp-Pro-Glu (amino acids 165-177), also contains the highly conserved pair of aspartic acid residues (positions 174 and 175), we investigated the contributions of this pair of acidic residues to binding of the c-Raf1 protein  in vitro.	bind
42391	1	9961	7	11	NULL	NULL	NULL	C-Raf1	GP		bind					Nef	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_25_15727_s_111	9624170	A Di-aspartic Acid Motif Is Critical for C-Raf1 Binding to Nef-- Since the carboxyl-terminal end of the Nef sequence deleted from the GST-delta41Nef fusion protein above, Leu-His-Pro-Val-Ser-Leu-His-Gly-Met-Asp-Asp-Pro-Glu (amino acids 165-177), also contains the highly conserved pair of aspartic acid residues (positions 174 and 175), we investigated the contributions of this pair of acidic residues to binding of the c-Raf1 protein  in vitro.	bind
42392	2	9961	7	11	NULL	NULL	NULL	Nef	GP		is critical for			Di-aspartic Acid Motif		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_25_15727_s_111	9624170	A Di-aspartic Acid Motif Is Critical for C-Raf1 Binding to Nef-- Since the carboxyl-terminal end of the Nef sequence deleted from the GST-delta41Nef fusion protein above, Leu-His-Pro-Val-Ser-Leu-His-Gly-Met-Asp-Asp-Pro-Glu (amino acids 165-177), also contains the highly conserved pair of aspartic acid residues (positions 174 and 175), we investigated the contributions of this pair of acidic residues to binding of the c-Raf1 protein  in vitro.	bind
34787	1	9962	6	11	NULL	NULL	NULL	DAB p3S5	GP		bind								KDR domain 1		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_19_14321_s_185	10799512	A diabody, DAB p3S5, which binds to KDR domain 1, was used in all ELISA to demonstrate the functional expression of the variant proteins and to normalize the amounts of protein added in the assay.	bind
49036	2	9962	6	11	NULL	NULL	NULL	DAB p3S5	GP		is a type of					diabody	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_19_14321_s_185	10799512	A diabody, DAB p3S5, which binds to KDR domain 1, was used in all ELISA to demonstrate the functional expression of the variant proteins and to normalize the amounts of protein added in the assay.	bind
42398	1	9962	7	11	NULL	NULL	NULL	DAB p3S5	GP		binds to								KDR domain 1		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_19_14321_s_185	10799512	A diabody, DAB p3S5, which binds to KDR domain 1, was used in all ELISA to demonstrate the functional expression of the variant proteins and to normalize the amounts of protein added in the assay.	bind
42399	2	9962	7	11	NULL	NULL	NULL	DAB p3S5	GP		is a type of					diabody	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_19_14321_s_185	10799512	A diabody, DAB p3S5, which binds to KDR domain 1, was used in all ELISA to demonstrate the functional expression of the variant proteins and to normalize the amounts of protein added in the assay.	bind
34788	1	9964	6	11	NULL	NULL	NULL	cortisol	Chemical		bind					hCBG	GP	native			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-mol-model-(online)_9_3_12733052_s_14	12733052	A difference accessible surface area (DASA) study revealed that cortisol  binds with the native hCBG more tightly than aldosterone.	bind
34789	2	9964	6	11	NULL	NULL	NULL	aldosterone	Chemical		bind					hCBG	GP	native			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-mol-model-(online)_9_3_12733052_s_14	12733052	A difference accessible surface area (DASA) study revealed that cortisol  binds with the native hCBG more tightly than aldosterone.	bind
34790	3	9964	6	11	NULL	NULL	NULL	statement 1	Process		more tightly than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-mol-model-(online)_9_3_12733052_s_14	12733052	A difference accessible surface area (DASA) study revealed that cortisol  binds with the native hCBG more tightly than aldosterone.	bind
42401	1	9964	7	11	NULL	NULL	NULL	cortisol	Chemical		binds					hCBG	GP	native			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-mol-model-(online)_9_3_12733052_s_14	12733052	A difference accessible surface area (DASA) study revealed that cortisol  binds with the native hCBG more tightly than aldosterone.	bind
42402	2	9964	7	11	NULL	NULL	NULL	aldosterone	Chemical		binds					hCBG	GP	native			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-mol-model-(online)_9_3_12733052_s_14	12733052	A difference accessible surface area (DASA) study revealed that cortisol  binds with the native hCBG more tightly than aldosterone.	bind
42403	3	9964	7	11	NULL	NULL	NULL	statement 1	Process		more tightly than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-mol-model-(online)_9_3_12733052_s_14	12733052	A difference accessible surface area (DASA) study revealed that cortisol  binds with the native hCBG more tightly than aldosterone.	bind
34791	1	9965	6	11	NULL	NULL	NULL	MTSET	Chemical		plays a role in					CFT	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_3_1608_s_195	10636852	A difference between the effects of the reagents on binding and transport is that the reaction of MTSET with Cys-90 or Cys-306 decreased the  K d of [3]CFT binding, whereas it increased the  Vmax of DA uptake.	bind
34792	2	9965	6	11	NULL	NULL	NULL	MTSET	Chemical		plays a role in					DA 	Chemical	uptake of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_3_1608_s_195	10636852	A difference between the effects of the reagents on binding and transport is that the reaction of MTSET with Cys-90 or Cys-306 decreased the  K d of [3]CFT binding, whereas it increased the  Vmax of DA uptake.	bind
42407	1	9965	7	11	NULL	NULL	NULL	MTSET	Chemical		plays a role in					CFT	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_3_1608_s_195	10636852	A difference between the effects of the reagents on binding and transport is that the reaction of MTSET with Cys-90 or Cys-306 decreased the  K d of [3]CFT binding, whereas it increased the  Vmax of DA uptake.	bind
42408	2	9965	7	11	NULL	NULL	NULL	MTSET	Chemical		plays a role in					DA	Chemical	uptake of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_3_1608_s_195	10636852	A difference between the effects of the reagents on binding and transport is that the reaction of MTSET with Cys-90 or Cys-306 decreased the  K d of [3]CFT binding, whereas it increased the  Vmax of DA uptake.	bind
34793	1	9966	6	11	NULL	NULL	NULL	band 3 tetramers	GP		promotes					cytoskeleton	CellComponent	binding of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_20_11771_s_113	11573011	A difference between the manner in which BS3 and DIDS act on band 3 is that the former shifts the band 3 population toward tetramers ( 25), which promotes cytoskeleton binding through band 3 binding with ankyrin, whereas the latter shifts the population of band 3 to dimers, which weakens cytoskeleton binding ( 26).	bind
34794	2	9966	6	11	NULL	NULL	NULL	band 3	GP		bind					ankyrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_20_11771_s_113	11573011	A difference between the manner in which BS3 and DIDS act on band 3 is that the former shifts the band 3 population toward tetramers ( 25), which promotes cytoskeleton binding through band 3 binding with ankyrin, whereas the latter shifts the population of band 3 to dimers, which weakens cytoskeleton binding ( 26).	bind
34795	3	9966	6	11	NULL	NULL	NULL	statement 1	Process		occurs through					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_20_11771_s_113	11573011	A difference between the manner in which BS3 and DIDS act on band 3 is that the former shifts the band 3 population toward tetramers ( 25), which promotes cytoskeleton binding through band 3 binding with ankyrin, whereas the latter shifts the population of band 3 to dimers, which weakens cytoskeleton binding ( 26).	bind
34796	4	9966	6	11	NULL	NULL	NULL	BS3	Chemical		increases 					band-3 tetramers	GP	formation of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_20_11771_s_113	11573011	A difference between the manner in which BS3 and DIDS act on band 3 is that the former shifts the band 3 population toward tetramers ( 25), which promotes cytoskeleton binding through band 3 binding with ankyrin, whereas the latter shifts the population of band 3 to dimers, which weakens cytoskeleton binding ( 26).	bind
34797	5	9966	6	11	NULL	NULL	NULL	DIDS	Chemical		promotes					band-3 dimers	GP	formation of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_20_11771_s_113	11573011	A difference between the manner in which BS3 and DIDS act on band 3 is that the former shifts the band 3 population toward tetramers ( 25), which promotes cytoskeleton binding through band 3 binding with ankyrin, whereas the latter shifts the population of band 3 to dimers, which weakens cytoskeleton binding ( 26).	bind
34798	6	9966	6	11	NULL	NULL	NULL	band 3 dimers	GP		weakens					cytoskeleton	CellComponent	binding of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_20_11771_s_113	11573011	A difference between the manner in which BS3 and DIDS act on band 3 is that the former shifts the band 3 population toward tetramers ( 25), which promotes cytoskeleton binding through band 3 binding with ankyrin, whereas the latter shifts the population of band 3 to dimers, which weakens cytoskeleton binding ( 26).	bind
42414	1	9966	7	11	NULL	NULL	NULL	band 3 tetramers	GP		promotes					cytoskeleton	CellComponent	binding of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_20_11771_s_113	11573011	A difference between the manner in which BS3 and DIDS act on band 3 is that the former shifts the band 3 population toward tetramers ( 25), which promotes cytoskeleton binding through band 3 binding with ankyrin, whereas the latter shifts the population of band 3 to dimers, which weakens cytoskeleton binding ( 26).	bind
42416	2	9966	7	11	NULL	NULL	NULL	band 3	GP		bind					ankyrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_20_11771_s_113	11573011	A difference between the manner in which BS3 and DIDS act on band 3 is that the former shifts the band 3 population toward tetramers ( 25), which promotes cytoskeleton binding through band 3 binding with ankyrin, whereas the latter shifts the population of band 3 to dimers, which weakens cytoskeleton binding ( 26).	bind
49044	3	9966	7	11	NULL	NULL	NULL	statement 1	Process		occurs through					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_20_11771_s_113	11573011	A difference between the manner in which BS3 and DIDS act on band 3 is that the former shifts the band 3 population toward tetramers ( 25), which promotes cytoskeleton binding through band 3 binding with ankyrin, whereas the latter shifts the population of band 3 to dimers, which weakens cytoskeleton binding ( 26).	bind
49045	4	9966	7	11	NULL	NULL	NULL	BS3	Chemical		increases					band-3 tetramers	GP	formation of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_20_11771_s_113	11573011	A difference between the manner in which BS3 and DIDS act on band 3 is that the former shifts the band 3 population toward tetramers ( 25), which promotes cytoskeleton binding through band 3 binding with ankyrin, whereas the latter shifts the population of band 3 to dimers, which weakens cytoskeleton binding ( 26).	bind
49046	5	9966	7	11	NULL	NULL	NULL	DIDS	Chemical		promotes					band-3 dimers	GP	formation of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_20_11771_s_113	11573011	A difference between the manner in which BS3 and DIDS act on band 3 is that the former shifts the band 3 population toward tetramers ( 25), which promotes cytoskeleton binding through band 3 binding with ankyrin, whereas the latter shifts the population of band 3 to dimers, which weakens cytoskeleton binding ( 26).	bind
49047	6	9966	7	11	NULL	NULL	NULL	band 3 dimers	GP		weakens					cytoskeleton	CellComponent	binding of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_20_11771_s_113	11573011	A difference between the manner in which BS3 and DIDS act on band 3 is that the former shifts the band 3 population toward tetramers ( 25), which promotes cytoskeleton binding through band 3 binding with ankyrin, whereas the latter shifts the population of band 3 to dimers, which weakens cytoskeleton binding ( 26).	bind
34799	1	9968	6	11	NULL	NULL	NULL	NGF	GP		bind					p75	GP				NULL	KA-treated adult animals	NULL	NULL	NULL	NULL	gw60_brainres_853_2_174_s_249	10640615	A difference between these two situations may be that in KA-treated adult animals, NGF binding to p75 produces cell death, whereas in developing animals, NGF promotes cell survival.	bind
34800	2	9968	6	11	NULL	NULL	NULL	statement 1	Process		produces					cell death	Process				NULL	KA-treated adult animals	NULL	NULL	NULL	NULL	gw60_brainres_853_2_174_s_249	10640615	A difference between these two situations may be that in KA-treated adult animals, NGF binding to p75 produces cell death, whereas in developing animals, NGF promotes cell survival.	bind
34801	3	9968	6	11	NULL	NULL	NULL	NGF	GP		promotes					cell survival	Process				NULL	developing animals	NULL	NULL	NULL	NULL	gw60_brainres_853_2_174_s_249	10640615	A difference between these two situations may be that in KA-treated adult animals, NGF binding to p75 produces cell death, whereas in developing animals, NGF promotes cell survival.	bind
42422	1	9968	7	11	NULL	NULL	NULL	NGF	GP		bind					p75	GP				NULL	KA-treated adult animals	NULL	NULL	NULL	NULL	gw60_brainres_853_2_174_s_249	10640615	A difference between these two situations may be that in KA-treated adult animals, NGF binding to p75 produces cell death, whereas in developing animals, NGF promotes cell survival.	bind
42423	2	9968	7	11	NULL	NULL	NULL	statement 1	Process		produces					cell death	Process				NULL	KA-treated adult animals	NULL	NULL	NULL	NULL	gw60_brainres_853_2_174_s_249	10640615	A difference between these two situations may be that in KA-treated adult animals, NGF binding to p75 produces cell death, whereas in developing animals, NGF promotes cell survival.	bind
42425	3	9968	7	11	NULL	NULL	NULL	NGF	GP		promotes					cell survival	Process				NULL	developing animals	NULL	NULL	NULL	NULL	gw60_brainres_853_2_174_s_249	10640615	A difference between these two situations may be that in KA-treated adult animals, NGF binding to p75 produces cell death, whereas in developing animals, NGF promotes cell survival.	bind
34813	1	9969	6	11	NULL	NULL	NULL	Ku proteins	GP		constitute					DNA-PK	GP				NULL	mammalian cells	NULL	NULL	NULL	NULL	gw60_genetics_148_3_975_s_324	9539418	A difference between yeast and mammalian cells is that in mammalian cells, the Ku proteins constitute the DNA-binding moiety of a larger complex, the DNA-dependent protein kinase (DNA-PK).	bind
49048	2	9969	6	11	NULL	NULL	NULL	DNA-PK	GP		is					DNA-dependent protein kinase 	GP				NULL		NULL	NULL	NULL	NULL	gw60_genetics_148_3_975_s_324	9539418	A difference between yeast and mammalian cells is that in mammalian cells, the Ku proteins constitute the DNA-binding moiety of a larger complex, the DNA-dependent protein kinase (DNA-PK).	bind
49049	3	9969	6	11	NULL	NULL	NULL	DNA-PK	GP		is a type of					DNA-binding moiety of a larger complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_genetics_148_3_975_s_324	9539418	A difference between yeast and mammalian cells is that in mammalian cells, the Ku proteins constitute the DNA-binding moiety of a larger complex, the DNA-dependent protein kinase (DNA-PK).	bind
42466	1	9969	7	11	NULL	NULL	NULL	 Ku proteins	GP		constitute					DNA-PK	GP				NULL	mammalian cells	NULL	NULL	NULL	NULL	gw60_genetics_148_3_975_s_324	9539418	A difference between yeast and mammalian cells is that in mammalian cells, the Ku proteins constitute the DNA-binding moiety of a larger complex, the DNA-dependent protein kinase (DNA-PK).	bind
42467	2	9969	7	11	NULL	NULL	NULL	DNA-PK	GP		is					DNA-dependent protein kinase 	GP				NULL		NULL	NULL	NULL	NULL	gw60_genetics_148_3_975_s_324	9539418	A difference between yeast and mammalian cells is that in mammalian cells, the Ku proteins constitute the DNA-binding moiety of a larger complex, the DNA-dependent protein kinase (DNA-PK).	bind
42468	3	9969	7	11	NULL	NULL	NULL	DNA-PK	GP		is a type of					DNA-binding moiety of a larger complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_genetics_148_3_975_s_324	9539418	A difference between yeast and mammalian cells is that in mammalian cells, the Ku proteins constitute the DNA-binding moiety of a larger complex, the DNA-dependent protein kinase (DNA-PK).	bind
34814	1	9970	6	11	NULL	NULL	NULL	CTD peptide	AminoAcid		bind					CID molecule	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_nature_430_6996_223_s_146	15241417	A difference Fourier for the peptide-soaked crystal was calculated  with phases from the CID model and identified strong density for the CTD peptide  bound to one CID molecule (chain B).	bind
42469	1	9970	7	11	NULL	NULL	NULL	CTD peptide	AminoAcid		bind					CID molecule	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_nature_430_6996_223_s_146	15241417	A difference Fourier for the peptide-soaked crystal was calculated  with phases from the CID model and identified strong density for the CTD peptide  bound to one CID molecule (chain B).	bind
34815	1	9971	6	11	NULL	NULL	NULL	VWF	GP		bind					rHPA-2a	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1302_s_121	12775575	A difference in affinity of VWF for rHPA-2a and rHPA-2b was also seen in the presence of 0.1 mug/mL botrocetin, where VWF bound with a Kd,app of 2.49 and 7.47 nmol/L to rHPA-2a and rHPA-2b, respectively (mean of 2 experiments), which could be confirmed with HPA-2a2a and HPA-2b2b platelets ( P<0.05) when anti-GPIbalpha moAb 27C11 was used as a reference to normalize for GPIbalpha numbers ( Figure 6).	bind
34816	2	9971	6	11	NULL	NULL	NULL	VWF	GP		bind					rHPA-2b	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1302_s_121	12775575	A difference in affinity of VWF for rHPA-2a and rHPA-2b was also seen in the presence of 0.1 mug/mL botrocetin, where VWF bound with a Kd,app of 2.49 and 7.47 nmol/L to rHPA-2a and rHPA-2b, respectively (mean of 2 experiments), which could be confirmed with HPA-2a2a and HPA-2b2b platelets ( P<0.05) when anti-GPIbalpha moAb 27C11 was used as a reference to normalize for GPIbalpha numbers ( Figure 6).	bind
34817	3	9971	6	11	NULL	NULL	NULL	statement 1	Process		occurs in presence of					botrocetin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1302_s_121	12775575	A difference in affinity of VWF for rHPA-2a and rHPA-2b was also seen in the presence of 0.1 mug/mL botrocetin, where VWF bound with a Kd,app of 2.49 and 7.47 nmol/L to rHPA-2a and rHPA-2b, respectively (mean of 2 experiments), which could be confirmed with HPA-2a2a and HPA-2b2b platelets ( P<0.05) when anti-GPIbalpha moAb 27C11 was used as a reference to normalize for GPIbalpha numbers ( Figure 6).	bind
34818	4	9971	6	11	NULL	NULL	NULL	statement 2	Process		occurs in presence of					botrocetin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1302_s_121	12775575	A difference in affinity of VWF for rHPA-2a and rHPA-2b was also seen in the presence of 0.1 mug/mL botrocetin, where VWF bound with a Kd,app of 2.49 and 7.47 nmol/L to rHPA-2a and rHPA-2b, respectively (mean of 2 experiments), which could be confirmed with HPA-2a2a and HPA-2b2b platelets ( P<0.05) when anti-GPIbalpha moAb 27C11 was used as a reference to normalize for GPIbalpha numbers ( Figure 6).	bind
42470	1	9971	7	11	NULL	NULL	NULL	VWF	GP		bind					rHPA-2a	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1302_s_121	12775575	A difference in affinity of VWF for rHPA-2a and rHPA-2b was also seen in the presence of 0.1 mug/mL botrocetin, where VWF bound with a Kd,app of 2.49 and 7.47 nmol/L to rHPA-2a and rHPA-2b, respectively (mean of 2 experiments), which could be confirmed with HPA-2a2a and HPA-2b2b platelets ( P<0.05) when anti-GPIbalpha moAb 27C11 was used as a reference to normalize for GPIbalpha numbers ( Figure 6).	bind
42471	2	9971	7	11	NULL	NULL	NULL	VWF	GP		bind					rHPA-2b	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1302_s_121	12775575	A difference in affinity of VWF for rHPA-2a and rHPA-2b was also seen in the presence of 0.1 mug/mL botrocetin, where VWF bound with a Kd,app of 2.49 and 7.47 nmol/L to rHPA-2a and rHPA-2b, respectively (mean of 2 experiments), which could be confirmed with HPA-2a2a and HPA-2b2b platelets ( P<0.05) when anti-GPIbalpha moAb 27C11 was used as a reference to normalize for GPIbalpha numbers ( Figure 6).	bind
42472	3	9971	7	11	NULL	NULL	NULL	statement 1	Process		in presence of					 botrocetin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1302_s_121	12775575	A difference in affinity of VWF for rHPA-2a and rHPA-2b was also seen in the presence of 0.1 mug/mL botrocetin, where VWF bound with a Kd,app of 2.49 and 7.47 nmol/L to rHPA-2a and rHPA-2b, respectively (mean of 2 experiments), which could be confirmed with HPA-2a2a and HPA-2b2b platelets ( P<0.05) when anti-GPIbalpha moAb 27C11 was used as a reference to normalize for GPIbalpha numbers ( Figure 6).	bind
42473	4	9971	7	11	NULL	NULL	NULL	statement 2	Process		in presence of					botrocetin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_7_1302_s_121	12775575	A difference in affinity of VWF for rHPA-2a and rHPA-2b was also seen in the presence of 0.1 mug/mL botrocetin, where VWF bound with a Kd,app of 2.49 and 7.47 nmol/L to rHPA-2a and rHPA-2b, respectively (mean of 2 experiments), which could be confirmed with HPA-2a2a and HPA-2b2b platelets ( P<0.05) when anti-GPIbalpha moAb 27C11 was used as a reference to normalize for GPIbalpha numbers ( Figure 6).	bind
42476	1	9972	7	NULL	NULL	0	NULL	Grb7	NULL		bind	NULL		SH2 domain		 HER 1-2 receptor	NULL	activated			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_21_12502_s_187	8647858	A difference in binding  selectivity between the Grb7 and Grb14 SH2 domains was more evident  when binding to the activated HER 1-2 receptor (an EGFR/ErbB2  chimera containing the intracellular domain of ErbB2) was investigated.	bind
42477	2	9972	7	NULL	NULL	0	NULL	Grb14 	NULL		bind	NULL		SH2 domain		HER 1-2 receptor	NULL	activated			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_21_12502_s_187	8647858	A difference in binding  selectivity between the Grb7 and Grb14 SH2 domains was more evident  when binding to the activated HER 1-2 receptor (an EGFR/ErbB2  chimera containing the intracellular domain of ErbB2) was investigated.	bind
42478	3	9972	7	10	NULL	0	NULL	HER 1-2 receptor	NULL		is	NULL				EGFR/ErbB2 chimera containing intracellular domain of ErbB2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_21_12502_s_187	8647858	A difference in binding  selectivity between the Grb7 and Grb14 SH2 domains was more evident  when binding to the activated HER 1-2 receptor (an EGFR/ErbB2  chimera containing the intracellular domain of ErbB2) was investigated.	bind
34821	1	9973	6	11	NULL	NULL	NULL	alpha-fetoprotein	GP	serum	bind					lectin	GP	lentil			NULL	hepatocellular carcinomas	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27810_s_18	8910378	A difference in the binding pattern of serum alpha-fetoprotein with lentil lectin between hepatocellular carcinomas and benign liver diseases has been reported ( 15,  16,  17).	bind
34822	2	9973	6	11	NULL	NULL	NULL	alpha-fetoprotein	GP	serum	bind					lectin	GP	lentil			NULL	benign liver diseases	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27810_s_18	8910378	A difference in the binding pattern of serum alpha-fetoprotein with lentil lectin between hepatocellular carcinomas and benign liver diseases has been reported ( 15,  16,  17).	bind
42479	1	9973	7	11	NULL	NULL	NULL	alpha-fetoprotein	GP	serum	bind					lectin	GP	lentil			NULL	hepatocellular carcinomas	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27810_s_18	8910378	A difference in the binding pattern of serum alpha-fetoprotein with lentil lectin between hepatocellular carcinomas and benign liver diseases has been reported ( 15,  16,  17).	bind
42480	2	9973	7	11	NULL	NULL	NULL	alpha-fetoprotein	GP	serum	bind					lectin	GP	lentil			NULL	benign liver diseases	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_44_27810_s_18	8910378	A difference in the binding pattern of serum alpha-fetoprotein with lentil lectin between hepatocellular carcinomas and benign liver diseases has been reported ( 15,  16,  17).	bind
34823	1	9974	6	11	NULL	NULL	NULL	dI	GP	isolated form of 	bind					NAD+/NADH	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_26_19490_s_308	10747934	A difference in the NAD+/NADH binding properties of dI in its isolated form and in the complete, membrane-bound protein was also inferred from a steady-state kinetic analysis ( 7).	bind
34824	2	9974	6	11	NULL	NULL	NULL	dI	GP	membrane-bound	bind					NAD+/NADH	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_26_19490_s_308	10747934	A difference in the NAD+/NADH binding properties of dI in its isolated form and in the complete, membrane-bound protein was also inferred from a steady-state kinetic analysis ( 7).	bind
42481	1	9974	7	11	NULL	NULL	NULL	NAD+/NADH	Chemical		bind					dI	GP	isolated form			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_26_19490_s_308	10747934	A difference in the NAD+/NADH binding properties of dI in its isolated form and in the complete, membrane-bound protein was also inferred from a steady-state kinetic analysis ( 7).	bind
42483	2	9974	7	11	NULL	NULL	NULL	NAD+/NADH	Chemical		bind					dI	GP	membrane-bound			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_26_19490_s_308	10747934	A difference in the NAD+/NADH binding properties of dI in its isolated form and in the complete, membrane-bound protein was also inferred from a steady-state kinetic analysis ( 7).	bind
34825	1	9976	6	11	NULL	NULL	NULL	tFR	GP		bind					FAD	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_37_23303_s_294	9287340	A difference spectrum between free FAD and tFR-bound FAD exhibits negative peaks at 490, 460, and 356 nm and a positive peak at 396 nm (Fig.  3,  curve C).	bind
42486	1	9976	7	11	NULL	NULL	NULL	 tFR	GP		bind					FAD	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_37_23303_s_294	9287340	A difference spectrum between free FAD and tFR-bound FAD exhibits negative peaks at 490, 460, and 356 nm and a positive peak at 396 nm (Fig.  3,  curve C).	bind
34826	1	9977	6	11	NULL	NULL	NULL	G-actin	GP	clevage of	diminishes			DNase-I-binding loop		actin	GP	rate of;; polymerization of 			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1478_1_138_s_98	10719182	A difference was observed in the rate of the polymerization-induced change: with intact actin, the maximum   n value was reached within 10-15 min, whereas with subtilisin-cleaved actin it took 25-30 min, in agreement with earlier observations showing that cleavage of G-actin within the DNase-I-binding loop diminishes the rate of actin polymerization [ 31 and  32].	bind
49052	2	9977	6	11	NULL	NULL	NULL	subtilisin	GP		cleaves					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1478_1_138_s_98	10719182	A difference was observed in the rate of the polymerization-induced change: with intact actin, the maximum   n value was reached within 10-15 min, whereas with subtilisin-cleaved actin it took 25-30 min, in agreement with earlier observations showing that cleavage of G-actin within the DNase-I-binding loop diminishes the rate of actin polymerization [ 31 and  32].	bind
42487	1	9977	7	11	NULL	NULL	NULL	subtilisin	GP		cleaves					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1478_1_138_s_98	10719182	A difference was observed in the rate of the polymerization-induced change: with intact actin, the maximum   n value was reached within 10-15 min, whereas with subtilisin-cleaved actin it took 25-30 min, in agreement with earlier observations showing that cleavage of G-actin within the DNase-I-binding loop diminishes the rate of actin polymerization [ 31 and  32].	bind
42488	2	9977	7	11	NULL	NULL	NULL	G-actin	GP	cleavage of	diminish			DNase-I-binding loop		actin	GP	 rate of;;polymerization of			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1478_1_138_s_98	10719182	A difference was observed in the rate of the polymerization-induced change: with intact actin, the maximum   n value was reached within 10-15 min, whereas with subtilisin-cleaved actin it took 25-30 min, in agreement with earlier observations showing that cleavage of G-actin within the DNase-I-binding loop diminishes the rate of actin polymerization [ 31 and  32].	bind
34827	1	9978	6	11	NULL	NULL	NULL	MAGE-3 peptide	GP		bind					HLA-A29	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_21_12463_s_226	8647853	A different and  more complex situation was observed for the MAGE-3 peptide binding by  HLA-A29.	bind
42489	1	9978	7	11	NULL	NULL	NULL	HLA-A29	GP		bind					MAGE-3 peptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_21_12463_s_226	8647853	A different and  more complex situation was observed for the MAGE-3 peptide binding by  HLA-A29.	bind
34828	1	9979	6	11	NULL	NULL	NULL	p22 phox	GP		bind			residues 176-195		p47 phox	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_300	11733522	A different approach to the identification of interaction domains in p22 phox was introduced by Kanegasaki and co-workers ( 44) who showed that a peptide corresponding to residues 176-195 of p22 phox inhibited SDS-induced NADPH oxidase activation in a cell-free system, albeit with a rather high IC50 (36 muM); the peptide also bound p47 phox in the presence of SDS.	bind
34829	2	9979	6	11	NULL	NULL	NULL	statement 1	Process		in the presence of					SDS	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_300	11733522	A different approach to the identification of interaction domains in p22 phox was introduced by Kanegasaki and co-workers ( 44) who showed that a peptide corresponding to residues 176-195 of p22 phox inhibited SDS-induced NADPH oxidase activation in a cell-free system, albeit with a rather high IC50 (36 muM); the peptide also bound p47 phox in the presence of SDS.	bind
34830	3	9979	6	11	NULL	NULL	NULL	SDS	Chemical		induces					NADPH oxidase	GP	activation of 			NULL	cell-free system	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_300	11733522	A different approach to the identification of interaction domains in p22 phox was introduced by Kanegasaki and co-workers ( 44) who showed that a peptide corresponding to residues 176-195 of p22 phox inhibited SDS-induced NADPH oxidase activation in a cell-free system, albeit with a rather high IC50 (36 muM); the peptide also bound p47 phox in the presence of SDS.	bind
34831	4	9979	6	11	NULL	NULL	NULL	p22 phox	GP		inhibits			residues 176-195		statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_300	11733522	A different approach to the identification of interaction domains in p22 phox was introduced by Kanegasaki and co-workers ( 44) who showed that a peptide corresponding to residues 176-195 of p22 phox inhibited SDS-induced NADPH oxidase activation in a cell-free system, albeit with a rather high IC50 (36 muM); the peptide also bound p47 phox in the presence of SDS.	bind
42490	1	9979	7	11	NULL	NULL	NULL	 SDS	Chemical		induce					NADPH oxidase 	GP	activation of			NULL	cell-free system	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_300	11733522	A different approach to the identification of interaction domains in p22 phox was introduced by Kanegasaki and co-workers ( 44) who showed that a peptide corresponding to residues 176-195 of p22 phox inhibited SDS-induced NADPH oxidase activation in a cell-free system, albeit with a rather high IC50 (36 muM); the peptide also bound p47 phox in the presence of SDS.	bind
42491	2	9979	7	11	NULL	NULL	NULL	p22 phox peptide	GP		inhibits			residues 176-195 		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_300	11733522	A different approach to the identification of interaction domains in p22 phox was introduced by Kanegasaki and co-workers ( 44) who showed that a peptide corresponding to residues 176-195 of p22 phox inhibited SDS-induced NADPH oxidase activation in a cell-free system, albeit with a rather high IC50 (36 muM); the peptide also bound p47 phox in the presence of SDS.	bind
42492	3	9979	7	11	NULL	NULL	NULL	p22 phox peptide	GP		bind			residues 176-195 		p47phox	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_300	11733522	A different approach to the identification of interaction domains in p22 phox was introduced by Kanegasaki and co-workers ( 44) who showed that a peptide corresponding to residues 176-195 of p22 phox inhibited SDS-induced NADPH oxidase activation in a cell-free system, albeit with a rather high IC50 (36 muM); the peptide also bound p47 phox in the presence of SDS.	bind
42493	4	9979	7	11	NULL	NULL	NULL	statement 3	Process		in the presence of					SDS	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_10_8421_s_300	11733522	A different approach to the identification of interaction domains in p22 phox was introduced by Kanegasaki and co-workers ( 44) who showed that a peptide corresponding to residues 176-195 of p22 phox inhibited SDS-induced NADPH oxidase activation in a cell-free system, albeit with a rather high IC50 (36 muM); the peptide also bound p47 phox in the presence of SDS.	bind
34832	1	9980	6	11	NULL	NULL	NULL	O2	Chemical		bind					Hb	GP	human;;adult			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_47_29859_s_11	8939926	A different behavior has been observed for O2 binding to human adult Hb, which displays some kinetic heterogeneity ( 3,  4,  5,  6).	bind
42494	1	9980	7	11	NULL	NULL	NULL	O2	Chemical		bind					Hb	GP	human;;adult			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_47_29859_s_11	8939926	A different behavior has been observed for O2 binding to human adult Hb, which displays some kinetic heterogeneity ( 3,  4,  5,  6).	bind
49061	1	9981	6	11	NULL	NULL	NULL	ligand	Chemical	endogenous	replaces					Fe(III) L116K CooAP	Chemical		Pro2		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_37_33616_s_155	12121986	A Different Endogenous Ligand Replaces Pro2 in Fe(III) L116K CooAP-- Given the close proximity of the position 116 residue to the heme and the unusually high aerobic DNA binding activity of L116K CooA, we expected that Fe(III) L116K would be structurally perturbed around the heme center and that this perturbation might be revealed by electronic absorption spectroscopy.	bind
49062	2	9981	6	11	NULL	NULL	NULL	CooA	Chemical		bind		aerobic	L116K		DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_37_33616_s_155	12121986	A Different Endogenous Ligand Replaces Pro2 in Fe(III) L116K CooAP-- Given the close proximity of the position 116 residue to the heme and the unusually high aerobic DNA binding activity of L116K CooA, we expected that Fe(III) L116K would be structurally perturbed around the heme center and that this perturbation might be revealed by electronic absorption spectroscopy.	bind
42584	1	9981	7	11	NULL	NULL	NULL	ligand	Chemical	endogenous	replaces					Fe(III) L116K CooAP	Chemical		Pro2		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_37_33616_s_155	12121986	A Different Endogenous Ligand Replaces Pro2 in Fe(III) L116K CooAP-- Given the close proximity of the position 116 residue to the heme and the unusually high aerobic DNA binding activity of L116K CooA, we expected that Fe(III) L116K would be structurally perturbed around the heme center and that this perturbation might be revealed by electronic absorption spectroscopy.	bind
42585	2	9981	7	11	NULL	NULL	NULL	CooA	Chemical		bind		aerobic	L116K		DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_37_33616_s_155	12121986	A Different Endogenous Ligand Replaces Pro2 in Fe(III) L116K CooAP-- Given the close proximity of the position 116 residue to the heme and the unusually high aerobic DNA binding activity of L116K CooA, we expected that Fe(III) L116K would be structurally perturbed around the heme center and that this perturbation might be revealed by electronic absorption spectroscopy.	bind
34833	1	9982	6	11	NULL	NULL	NULL	initiation factor 4E	GP		bind					5' RNA cap	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_12_3875_s_308	11739787	A different labeling was observed with antibodies to initiation factor 4E, a protein that binds to the 5' RNA cap and mediates ribosome binding (Sonenberg  et al., 1978  ).	bind
34834	2	9982	6	11	NULL	NULL	NULL	statement 1	Process		mediates					ribosome	CellComponent	binding of 			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_12_3875_s_308	11739787	A different labeling was observed with antibodies to initiation factor 4E, a protein that binds to the 5' RNA cap and mediates ribosome binding (Sonenberg  et al., 1978  ).	bind
42587	1	9982	7	11	NULL	NULL	NULL	initiation factor 4E	GP		bind					5' RNA cap	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_12_3875_s_308	11739787	A different labeling was observed with antibodies to initiation factor 4E, a protein that binds to the 5' RNA cap and mediates ribosome binding (Sonenberg  et al., 1978  ).	bind
42588	2	9982	7	11	NULL	NULL	NULL	statement 1	Process		mediates					ribosome	CellComponent	binding of			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_12_3875_s_308	11739787	A different labeling was observed with antibodies to initiation factor 4E, a protein that binds to the 5' RNA cap and mediates ribosome binding (Sonenberg  et al., 1978  ).	bind
34984	1	9983	6	11	NULL	NULL	NULL	p12I	GP	 cytoplasm facing region	bind					calcineurin	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_311_4_1117_s_125	14623298	A different region of p12I, presumably facing the cytoplasm, binds calcineurin; however, the SPSLPLT sequence  in this region is a relatively poor PxIxIT motif since it contains an internal proline  and since substitution of the essential threonine with alanine does not impair binding  of p12I to calcineurin [  40].	bind
34985	2	9983	6	11	NULL	NULL	NULL	p12I	GP		is a type of		relatively	SPSLPLT sequence				poor	PxIxIT motif		NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_311_4_1117_s_125	14623298	A different region of p12I, presumably facing the cytoplasm, binds calcineurin; however, the SPSLPLT sequence  in this region is a relatively poor PxIxIT motif since it contains an internal proline  and since substitution of the essential threonine with alanine does not impair binding  of p12I to calcineurin [  40].	bind
34986	3	9983	6	11	NULL	NULL	NULL				is substituted with			threonine in PxIxIT motif					alanine in PxIxIT motif		NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_311_4_1117_s_125	14623298	A different region of p12I, presumably facing the cytoplasm, binds calcineurin; however, the SPSLPLT sequence  in this region is a relatively poor PxIxIT motif since it contains an internal proline  and since substitution of the essential threonine with alanine does not impair binding  of p12I to calcineurin [  40].	bind
34987	4	9983	6	11	NULL	NULL	NULL	statement 3	Process		does not impair					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_311_4_1117_s_125	14623298	A different region of p12I, presumably facing the cytoplasm, binds calcineurin; however, the SPSLPLT sequence  in this region is a relatively poor PxIxIT motif since it contains an internal proline  and since substitution of the essential threonine with alanine does not impair binding  of p12I to calcineurin [  40].	bind
42589	1	9983	7	11	NULL	NULL	NULL	 p12I 	GP	cytoplasm facing region	binds					calcineurin	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_311_4_1117_s_125	14623298	A different region of p12I, presumably facing the cytoplasm, binds calcineurin; however, the SPSLPLT sequence  in this region is a relatively poor PxIxIT motif since it contains an internal proline  and since substitution of the essential threonine with alanine does not impair binding  of p12I to calcineurin [  40].	bind
42590	2	9983	7	11	NULL	NULL	NULL	p12I	GP		is a type of			SPSLPLT sequence					PxIxIT motif		NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_311_4_1117_s_125	14623298	A different region of p12I, presumably facing the cytoplasm, binds calcineurin; however, the SPSLPLT sequence  in this region is a relatively poor PxIxIT motif since it contains an internal proline  and since substitution of the essential threonine with alanine does not impair binding  of p12I to calcineurin [  40].	bind
42591	3	9983	7	11	NULL	NULL	NULL	statement 2	Process		is because of 					internal proline residue	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_311_4_1117_s_125	14623298	A different region of p12I, presumably facing the cytoplasm, binds calcineurin; however, the SPSLPLT sequence  in this region is a relatively poor PxIxIT motif since it contains an internal proline  and since substitution of the essential threonine with alanine does not impair binding  of p12I to calcineurin [  40].	bind
42592	4	9983	7	11	NULL	NULL	NULL				is substituted with			threonine in PxIxIT motif					alanine in PxIxIT motif		NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_311_4_1117_s_125	14623298	A different region of p12I, presumably facing the cytoplasm, binds calcineurin; however, the SPSLPLT sequence  in this region is a relatively poor PxIxIT motif since it contains an internal proline  and since substitution of the essential threonine with alanine does not impair binding  of p12I to calcineurin [  40].	bind
42593	5	9983	7	11	NULL	NULL	NULL	statement 4	Process		does not impair					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_311_4_1117_s_125	14623298	A different region of p12I, presumably facing the cytoplasm, binds calcineurin; however, the SPSLPLT sequence  in this region is a relatively poor PxIxIT motif since it contains an internal proline  and since substitution of the essential threonine with alanine does not impair binding  of p12I to calcineurin [  40].	bind
34835	1	9984	6	11	NULL	NULL	NULL	PlexB	GP		bind					RhoA	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_1_39_s_6	11604137	A different region of PlexB binds to RhoA.	bind
42594	1	9984	7	11	NULL	NULL	NULL	PlexB	GP		binds to					RhoA	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_1_39_s_6	11604137	A different region of PlexB binds to RhoA.	bind
34988	1	9985	6	11	NULL	NULL	NULL	V1ROSS proteins	GP		bind					calmodulin	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_mol-pharmacol_70_1_16574744_s_8	16574744	A different series of soluble receptor analogs,  named vasopressin receptor 1 elements on a soluble scaffold (V1ROSS) proteins,  consist of the third intracellular loop and/or the C-terminal segment  of the hV1R receptor juxtaposed on the surface of the MBP. V1ROSS proteins  bind calmodulin and a truncated, phosphorylation-independent form of arrestin2  more tightly than the corresponding linear fusion proteins.	bind
34989	2	9985	6	11	NULL	NULL	NULL	V1ROSS proteins	GP		bind					arrestin2	GP	truncated;; phosphorylation-independent form of			NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_mol-pharmacol_70_1_16574744_s_8	16574744	A different series of soluble receptor analogs,  named vasopressin receptor 1 elements on a soluble scaffold (V1ROSS) proteins,  consist of the third intracellular loop and/or the C-terminal segment  of the hV1R receptor juxtaposed on the surface of the MBP. V1ROSS proteins  bind calmodulin and a truncated, phosphorylation-independent form of arrestin2  more tightly than the corresponding linear fusion proteins.	bind
34990	3	9985	6	11	NULL	NULL	NULL	V1ROSS proteins	GP		bind					arrestin2	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_mol-pharmacol_70_1_16574744_s_8	16574744	A different series of soluble receptor analogs,  named vasopressin receptor 1 elements on a soluble scaffold (V1ROSS) proteins,  consist of the third intracellular loop and/or the C-terminal segment  of the hV1R receptor juxtaposed on the surface of the MBP. V1ROSS proteins  bind calmodulin and a truncated, phosphorylation-independent form of arrestin2  more tightly than the corresponding linear fusion proteins.	bind
34991	4	9985	6	11	NULL	NULL	NULL	statement 1	Process	affinity of	is more than					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_mol-pharmacol_70_1_16574744_s_8	16574744	A different series of soluble receptor analogs,  named vasopressin receptor 1 elements on a soluble scaffold (V1ROSS) proteins,  consist of the third intracellular loop and/or the C-terminal segment  of the hV1R receptor juxtaposed on the surface of the MBP. V1ROSS proteins  bind calmodulin and a truncated, phosphorylation-independent form of arrestin2  more tightly than the corresponding linear fusion proteins.	bind
34992	5	9985	6	11	NULL	NULL	NULL	V1ROSS	GP		is					vasopressin receptor 1 elements on a soluble scaffold	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_mol-pharmacol_70_1_16574744_s_8	16574744	A different series of soluble receptor analogs,  named vasopressin receptor 1 elements on a soluble scaffold (V1ROSS) proteins,  consist of the third intracellular loop and/or the C-terminal segment  of the hV1R receptor juxtaposed on the surface of the MBP. V1ROSS proteins  bind calmodulin and a truncated, phosphorylation-independent form of arrestin2  more tightly than the corresponding linear fusion proteins.	bind
34993	6	9985	6	11	NULL	NULL	NULL	V1ROSS protein	GP		is a type of					receptor analog	GP	soluble			NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_mol-pharmacol_70_1_16574744_s_8	16574744	A different series of soluble receptor analogs,  named vasopressin receptor 1 elements on a soluble scaffold (V1ROSS) proteins,  consist of the third intracellular loop and/or the C-terminal segment  of the hV1R receptor juxtaposed on the surface of the MBP. V1ROSS proteins  bind calmodulin and a truncated, phosphorylation-independent form of arrestin2  more tightly than the corresponding linear fusion proteins.	bind
34994	7	9985	6	11	NULL	NULL	NULL	V1ROSS proteins	GP		consists of					hV1R receptor	GP		third intracellular loop		NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_mol-pharmacol_70_1_16574744_s_8	16574744	A different series of soluble receptor analogs,  named vasopressin receptor 1 elements on a soluble scaffold (V1ROSS) proteins,  consist of the third intracellular loop and/or the C-terminal segment  of the hV1R receptor juxtaposed on the surface of the MBP. V1ROSS proteins  bind calmodulin and a truncated, phosphorylation-independent form of arrestin2  more tightly than the corresponding linear fusion proteins.	bind
34995	8	9985	6	11	NULL	NULL	NULL	V1ROSS protein	GP		consists of					hV1R receptor juxtaposed on the surface of the MBP	GP		C-terminal segment		NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_mol-pharmacol_70_1_16574744_s_8	16574744	A different series of soluble receptor analogs,  named vasopressin receptor 1 elements on a soluble scaffold (V1ROSS) proteins,  consist of the third intracellular loop and/or the C-terminal segment  of the hV1R receptor juxtaposed on the surface of the MBP. V1ROSS proteins  bind calmodulin and a truncated, phosphorylation-independent form of arrestin2  more tightly than the corresponding linear fusion proteins.	bind
42595	1	9985	7	11	NULL	NULL	NULL	vasopressin receptor 1 elements	GP		present on					V1ROSS proteins	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_mol-pharmacol_70_1_16574744_s_8	16574744	A different series of soluble receptor analogs,  named vasopressin receptor 1 elements on a soluble scaffold (V1ROSS) proteins,  consist of the third intracellular loop and/or the C-terminal segment  of the hV1R receptor juxtaposed on the surface of the MBP. V1ROSS proteins  bind calmodulin and a truncated, phosphorylation-independent form of arrestin2  more tightly than the corresponding linear fusion proteins.	bind
42596	2	9985	7	11	NULL	NULL	NULL	statement 1	Process		consist of					hV1R receptor	GP		third intracellular loop		NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_mol-pharmacol_70_1_16574744_s_8	16574744	A different series of soluble receptor analogs,  named vasopressin receptor 1 elements on a soluble scaffold (V1ROSS) proteins,  consist of the third intracellular loop and/or the C-terminal segment  of the hV1R receptor juxtaposed on the surface of the MBP. V1ROSS proteins  bind calmodulin and a truncated, phosphorylation-independent form of arrestin2  more tightly than the corresponding linear fusion proteins.	bind
42597	3	9985	7	11	NULL	NULL	NULL	statement 1	Process		consist of					hV1R receptor	GP		C-terminal segment 		NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_mol-pharmacol_70_1_16574744_s_8	16574744	A different series of soluble receptor analogs,  named vasopressin receptor 1 elements on a soluble scaffold (V1ROSS) proteins,  consist of the third intracellular loop and/or the C-terminal segment  of the hV1R receptor juxtaposed on the surface of the MBP. V1ROSS proteins  bind calmodulin and a truncated, phosphorylation-independent form of arrestin2  more tightly than the corresponding linear fusion proteins.	bind
42598	4	9985	7	11	NULL	NULL	NULL	statement 2	Process		 juxtaposed on					MBP	GP	surface of			NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_mol-pharmacol_70_1_16574744_s_8	16574744	A different series of soluble receptor analogs,  named vasopressin receptor 1 elements on a soluble scaffold (V1ROSS) proteins,  consist of the third intracellular loop and/or the C-terminal segment  of the hV1R receptor juxtaposed on the surface of the MBP. V1ROSS proteins  bind calmodulin and a truncated, phosphorylation-independent form of arrestin2  more tightly than the corresponding linear fusion proteins.	bind
42599	5	9985	7	11	NULL	NULL	NULL	statement 3	Process		juxtaposed on					MBP	GP	surface of			NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_mol-pharmacol_70_1_16574744_s_8	16574744	A different series of soluble receptor analogs,  named vasopressin receptor 1 elements on a soluble scaffold (V1ROSS) proteins,  consist of the third intracellular loop and/or the C-terminal segment  of the hV1R receptor juxtaposed on the surface of the MBP. V1ROSS proteins  bind calmodulin and a truncated, phosphorylation-independent form of arrestin2  more tightly than the corresponding linear fusion proteins.	bind
42600	6	9985	7	11	NULL	NULL	NULL	V1ROSS proteins	GP		bind					calmodulin 	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_mol-pharmacol_70_1_16574744_s_8	16574744	A different series of soluble receptor analogs,  named vasopressin receptor 1 elements on a soluble scaffold (V1ROSS) proteins,  consist of the third intracellular loop and/or the C-terminal segment  of the hV1R receptor juxtaposed on the surface of the MBP. V1ROSS proteins  bind calmodulin and a truncated, phosphorylation-independent form of arrestin2  more tightly than the corresponding linear fusion proteins.	bind
42601	7	9985	7	11	NULL	NULL	NULL	V1ROSS proteins	GP		bind					arrestin2	GP	truncated;;phosphorylation-independent form of 			NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_mol-pharmacol_70_1_16574744_s_8	16574744	A different series of soluble receptor analogs,  named vasopressin receptor 1 elements on a soluble scaffold (V1ROSS) proteins,  consist of the third intracellular loop and/or the C-terminal segment  of the hV1R receptor juxtaposed on the surface of the MBP. V1ROSS proteins  bind calmodulin and a truncated, phosphorylation-independent form of arrestin2  more tightly than the corresponding linear fusion proteins.	bind
42602	8	9985	7	11	NULL	NULL	NULL	V1ROSS proteins	GP		bind					linear fusion protein	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_mol-pharmacol_70_1_16574744_s_8	16574744	A different series of soluble receptor analogs,  named vasopressin receptor 1 elements on a soluble scaffold (V1ROSS) proteins,  consist of the third intracellular loop and/or the C-terminal segment  of the hV1R receptor juxtaposed on the surface of the MBP. V1ROSS proteins  bind calmodulin and a truncated, phosphorylation-independent form of arrestin2  more tightly than the corresponding linear fusion proteins.	bind
42603	9	9985	7	11	NULL	NULL	NULL	statement 6	Process		is more tight than					statement 8	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_mol-pharmacol_70_1_16574744_s_8	16574744	A different series of soluble receptor analogs,  named vasopressin receptor 1 elements on a soluble scaffold (V1ROSS) proteins,  consist of the third intracellular loop and/or the C-terminal segment  of the hV1R receptor juxtaposed on the surface of the MBP. V1ROSS proteins  bind calmodulin and a truncated, phosphorylation-independent form of arrestin2  more tightly than the corresponding linear fusion proteins.	bind
42604	10	9985	7	11	NULL	NULL	NULL	statement 7	Process		is more tight than					statement 8	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_mol-pharmacol_70_1_16574744_s_8	16574744	A different series of soluble receptor analogs,  named vasopressin receptor 1 elements on a soluble scaffold (V1ROSS) proteins,  consist of the third intracellular loop and/or the C-terminal segment  of the hV1R receptor juxtaposed on the surface of the MBP. V1ROSS proteins  bind calmodulin and a truncated, phosphorylation-independent form of arrestin2  more tightly than the corresponding linear fusion proteins.	bind
42605	11	9985	7	11	NULL	NULL	NULL	V1ROSS proteins	GP		is a type of					soluble scaffold proteins	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_mol-pharmacol_70_1_16574744_s_8	16574744	A different series of soluble receptor analogs,  named vasopressin receptor 1 elements on a soluble scaffold (V1ROSS) proteins,  consist of the third intracellular loop and/or the C-terminal segment  of the hV1R receptor juxtaposed on the surface of the MBP. V1ROSS proteins  bind calmodulin and a truncated, phosphorylation-independent form of arrestin2  more tightly than the corresponding linear fusion proteins.	bind
34836	1	9987	6	11	NULL	NULL	NULL	[BeF3]ADP	Chemical		bind					NS3h	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_26_23311_s_155	12660239	A different type of fluorimetric titration was conducted to confirm that  [BeF3]ADP binding to NS3h indeed reduces its affinity for ssDNA.	bind
34837	2	9987	6	11	NULL	NULL	NULL	NS3h	GP		has affinity for					ssDNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_26_23311_s_155	12660239	A different type of fluorimetric titration was conducted to confirm that  [BeF3]ADP binding to NS3h indeed reduces its affinity for ssDNA.	bind
34838	3	9987	6	11	NULL	NULL	NULL	statement 1	Process		reduces					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_26_23311_s_155	12660239	A different type of fluorimetric titration was conducted to confirm that  [BeF3]ADP binding to NS3h indeed reduces its affinity for ssDNA.	bind
42606	1	9987	7	11	NULL	NULL	NULL	 [BeF3]ADP	Chemical		bind					NS3h	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_26_23311_s_155	12660239	A different type of fluorimetric titration was conducted to confirm that  [BeF3]ADP binding to NS3h indeed reduces its affinity for ssDNA.	bind
42607	2	9987	7	11	NULL	NULL	NULL	NS3h	GP		affinity for					ssDNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_26_23311_s_155	12660239	A different type of fluorimetric titration was conducted to confirm that  [BeF3]ADP binding to NS3h indeed reduces its affinity for ssDNA.	bind
42608	3	9987	7	11	NULL	NULL	NULL	statement 1	Process		reduces					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_26_23311_s_155	12660239	A different type of fluorimetric titration was conducted to confirm that  [BeF3]ADP binding to NS3h indeed reduces its affinity for ssDNA.	bind
34839	1	9989	6	11	NULL	NULL	NULL	O2	Chemical		bind					deoxyhemoglobin	GP				NULL	erythrocytes	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_30_18709_s_86	9668042	A Diffusion Model for Reaction of Free NO with RBCs-- Hartridge and Roughton ( 8) reported in 1927 that reaction (binding) of O2 with deoxyhemoglobin occurs much more slowly when the deoxyhemoglobin is contained within erythrocytes than when free in solution.	bind
34840	2	9989	6	11	NULL	NULL	NULL	O2	Chemical		bind					erythrocytes	Cell	free			NULL	solution	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_30_18709_s_86	9668042	A Diffusion Model for Reaction of Free NO with RBCs-- Hartridge and Roughton ( 8) reported in 1927 that reaction (binding) of O2 with deoxyhemoglobin occurs much more slowly when the deoxyhemoglobin is contained within erythrocytes than when free in solution.	bind
34841	3	9989	6	11	NULL	NULL	NULL	statement 1	Process		slower than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_30_18709_s_86	9668042	A Diffusion Model for Reaction of Free NO with RBCs-- Hartridge and Roughton ( 8) reported in 1927 that reaction (binding) of O2 with deoxyhemoglobin occurs much more slowly when the deoxyhemoglobin is contained within erythrocytes than when free in solution.	bind
57124	4	9989	6	11	NULL	NULL	NULL	NO	Chemical	free	reacts with					RBCs	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_30_18709_s_86	9668042	A Diffusion Model for Reaction of Free NO with RBCs-- Hartridge and Roughton ( 8) reported in 1927 that reaction (binding) of O2 with deoxyhemoglobin occurs much more slowly when the deoxyhemoglobin is contained within erythrocytes than when free in solution.	bind
42609	1	9989	7	11	NULL	NULL	NULL	NO 	Chemical	free	reacts with					RBCs	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_30_18709_s_86	9668042	A Diffusion Model for Reaction of Free NO with RBCs-- Hartridge and Roughton ( 8) reported in 1927 that reaction (binding) of O2 with deoxyhemoglobin occurs much more slowly when the deoxyhemoglobin is contained within erythrocytes than when free in solution.	bind
42610	2	9989	7	11	NULL	NULL	NULL	O2	Chemical		binds					deoxyhemoglobin	GP				NULL	erythrocytes	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_30_18709_s_86	9668042	A Diffusion Model for Reaction of Free NO with RBCs-- Hartridge and Roughton ( 8) reported in 1927 that reaction (binding) of O2 with deoxyhemoglobin occurs much more slowly when the deoxyhemoglobin is contained within erythrocytes than when free in solution.	bind
42611	3	9989	7	11	NULL	NULL	NULL	O2	Chemical		binds					deoxyhemoglobin	GP	free			NULL	solution	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_30_18709_s_86	9668042	A Diffusion Model for Reaction of Free NO with RBCs-- Hartridge and Roughton ( 8) reported in 1927 that reaction (binding) of O2 with deoxyhemoglobin occurs much more slowly when the deoxyhemoglobin is contained within erythrocytes than when free in solution.	bind
42612	4	9989	7	11	NULL	NULL	NULL	statement 2	Process		is slower than					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_30_18709_s_86	9668042	A Diffusion Model for Reaction of Free NO with RBCs-- Hartridge and Roughton ( 8) reported in 1927 that reaction (binding) of O2 with deoxyhemoglobin occurs much more slowly when the deoxyhemoglobin is contained within erythrocytes than when free in solution.	bind
34842	1	9991	6	11	NULL	NULL	NULL	FGF-2	GP		bind					SOS	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_26_16382_s_150	9195945	A dimer formed by simultaneous binding of two FGF-2s to one SOS would thus be a head to head dimer where FGF-2 molecules are  trans to the SOS ligand (Fig.  4 A), with SOS presenting two anionic surfaces for binding.	bind
42614	1	9991	7	11	NULL	NULL	NULL	FGF-2	GP		bind					SOS	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_26_16382_s_150	9195945	A dimer formed by simultaneous binding of two FGF-2s to one SOS would thus be a head to head dimer where FGF-2 molecules are  trans to the SOS ligand (Fig.  4 A), with SOS presenting two anionic surfaces for binding.	bind
35078	1	9992	6	11	NULL	NULL	NULL	E2	GP		bind							proximal		E2 BS12	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3522_s_418	10652347	A dimer of E1 is first recruited to the E1-binding site by cooperative interactions with E2 bound to proximal E2 BS12 ( 13) or distal BS11.2 Sequences in the E1 palindrome are critical for dimer binding.	bind
35079	2	9992	6	11	NULL	NULL	NULL	E2	GP		bind							distal		BS11.2 Sequences in E1 palindrome	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3522_s_418	10652347	A dimer of E1 is first recruited to the E1-binding site by cooperative interactions with E2 bound to proximal E2 BS12 ( 13) or distal BS11.2 Sequences in the E1 palindrome are critical for dimer binding.	bind
35080	3	9992	6	11	NULL	NULL	NULL	E1 dimer	GP		is recruited to									E1-binding site	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3522_s_418	10652347	A dimer of E1 is first recruited to the E1-binding site by cooperative interactions with E2 bound to proximal E2 BS12 ( 13) or distal BS11.2 Sequences in the E1 palindrome are critical for dimer binding.	bind
35081	4	9992	6	11	NULL	NULL	NULL	E1 dimer	GP		interacts with		cooperatively			statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3522_s_418	10652347	A dimer of E1 is first recruited to the E1-binding site by cooperative interactions with E2 bound to proximal E2 BS12 ( 13) or distal BS11.2 Sequences in the E1 palindrome are critical for dimer binding.	bind
35082	5	9992	6	11	NULL	NULL	NULL	E1 dimer	GP		interacts with		cooperatively			statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3522_s_418	10652347	A dimer of E1 is first recruited to the E1-binding site by cooperative interactions with E2 bound to proximal E2 BS12 ( 13) or distal BS11.2 Sequences in the E1 palindrome are critical for dimer binding.	bind
35083	6	9992	6	11	NULL	NULL	NULL	statement 3	Process		occurs via					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3522_s_418	10652347	A dimer of E1 is first recruited to the E1-binding site by cooperative interactions with E2 bound to proximal E2 BS12 ( 13) or distal BS11.2 Sequences in the E1 palindrome are critical for dimer binding.	bind
35084	7	9992	6	11	NULL	NULL	NULL	statement 3	Process		occurs via					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3522_s_418	10652347	A dimer of E1 is first recruited to the E1-binding site by cooperative interactions with E2 bound to proximal E2 BS12 ( 13) or distal BS11.2 Sequences in the E1 palindrome are critical for dimer binding.	bind
35085	8	9992	6	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3522_s_418	10652347	A dimer of E1 is first recruited to the E1-binding site by cooperative interactions with E2 bound to proximal E2 BS12 ( 13) or distal BS11.2 Sequences in the E1 palindrome are critical for dimer binding.	bind
42619	1	9992	7	11	NULL	NULL	NULL	E1 dimer	GP		recruits to									E1-binding site	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3522_s_418	10652347	A dimer of E1 is first recruited to the E1-binding site by cooperative interactions with E2 bound to proximal E2 BS12 ( 13) or distal BS11.2 Sequences in the E1 palindrome are critical for dimer binding.	bind
42622	2	9992	7	11	NULL	NULL	NULL	E2	GP		bind							proximal		E2 BS12	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3522_s_418	10652347	A dimer of E1 is first recruited to the E1-binding site by cooperative interactions with E2 bound to proximal E2 BS12 ( 13) or distal BS11.2 Sequences in the E1 palindrome are critical for dimer binding.	bind
42623	3	9992	7	11	NULL	NULL	NULL	E2	GP		bind							distal		BS11.2 sequences in E1 palindrome	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3522_s_418	10652347	A dimer of E1 is first recruited to the E1-binding site by cooperative interactions with E2 bound to proximal E2 BS12 ( 13) or distal BS11.2 Sequences in the E1 palindrome are critical for dimer binding.	bind
42624	4	9992	7	11	NULL	NULL	NULL	E1 dimer	GP		interacts with		cooperatively			statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3522_s_418	10652347	A dimer of E1 is first recruited to the E1-binding site by cooperative interactions with E2 bound to proximal E2 BS12 ( 13) or distal BS11.2 Sequences in the E1 palindrome are critical for dimer binding.	bind
42637	5	9992	7	11	NULL	NULL	NULL	E1 dimer	GP		interacts with		cooperatively			statement 3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3522_s_418	10652347	A dimer of E1 is first recruited to the E1-binding site by cooperative interactions with E2 bound to proximal E2 BS12 ( 13) or distal BS11.2 Sequences in the E1 palindrome are critical for dimer binding.	bind
42638	6	9992	7	11	NULL	NULL	NULL	statement 1	Process		occurs via					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3522_s_418	10652347	A dimer of E1 is first recruited to the E1-binding site by cooperative interactions with E2 bound to proximal E2 BS12 ( 13) or distal BS11.2 Sequences in the E1 palindrome are critical for dimer binding.	bind
49148	7	9992	7	11	NULL	NULL	NULL	statement 1	Process		occurs via					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3522_s_418	10652347	A dimer of E1 is first recruited to the E1-binding site by cooperative interactions with E2 bound to proximal E2 BS12 ( 13) or distal BS11.2 Sequences in the E1 palindrome are critical for dimer binding.	bind
57125	8	9992	7	11	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3522_s_418	10652347	A dimer of E1 is first recruited to the E1-binding site by cooperative interactions with E2 bound to proximal E2 BS12 ( 13) or distal BS11.2 Sequences in the E1 palindrome are critical for dimer binding.	bind
34843	1	9993	6	11	NULL	NULL	NULL	EBNA1 dimer	GP		bind									18 bp binding site	NULL		NULL	NULL	NULL	NULL	gw60_cell_84_5_791_s_66	8625416	A Dimer of EBNA1 Bound to Its  18 bp Binding Site	bind
42639	1	9993	7	11	NULL	NULL	NULL	 EBNA1 dimer	GP		bind									18 bp Binding Site	NULL		NULL	NULL	NULL	NULL	gw60_cell_84_5_791_s_66	8625416	A Dimer of EBNA1 Bound to Its  18 bp Binding Site	bind
34844	1	9994	6	11	NULL	NULL	NULL	EBNA1 dimer	GP		bind									18 bp recognition site	NULL		NULL	NULL	NULL	NULL	gw60_cell_84_5_791_s_201	8625416	A dimer of EBNA1 bound to its 18 bp recognition site cannot  function as an origin.	bind
34845	2	9994	6	11	NULL	NULL	NULL	EBNA1 dimer	GP		does not function as 					origin	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_84_5_791_s_201	8625416	A dimer of EBNA1 bound to its 18 bp recognition site cannot  function as an origin.	bind
42640	1	9994	7	11	NULL	NULL	NULL	EBNA1 dimer	GP		bind									18 bp recognition site	NULL		NULL	NULL	NULL	NULL	gw60_cell_84_5_791_s_201	8625416	A dimer of EBNA1 bound to its 18 bp recognition site cannot  function as an origin.	bind
42641	2	9994	7	11	NULL	NULL	NULL	statement 1	GP		does not function as					origin	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_cell_84_5_791_s_201	8625416	A dimer of EBNA1 bound to its 18 bp recognition site cannot  function as an origin.	bind
34846	1	9995	6	11	NULL	NULL	NULL	PICK1 dimer	GP		bind					PKC receptor subunit	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_6_919_s_131	10727702	A dimer of PICK1 could bind to both PKC  and AMPA receptor subunits, bringing active PKC  into intimate contact with the AMPA receptor.	bind
34847	2	9995	6	11	NULL	NULL	NULL	PICK1 dimer	GP		bind					AMPA receptor subunit	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_6_919_s_131	10727702	A dimer of PICK1 could bind to both PKC  and AMPA receptor subunits, bringing active PKC  into intimate contact with the AMPA receptor.	bind
34848	3	9995	6	11	NULL	NULL	NULL	PKC	GP	active	contact with		intimate			AMPA receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_6_919_s_131	10727702	A dimer of PICK1 could bind to both PKC  and AMPA receptor subunits, bringing active PKC  into intimate contact with the AMPA receptor.	bind
34849	4	9995	6	11	NULL	NULL	NULL	statement 1	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_6_919_s_131	10727702	A dimer of PICK1 could bind to both PKC  and AMPA receptor subunits, bringing active PKC  into intimate contact with the AMPA receptor.	bind
34850	5	9995	6	11	NULL	NULL	NULL	statement 2	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_6_919_s_131	10727702	A dimer of PICK1 could bind to both PKC  and AMPA receptor subunits, bringing active PKC  into intimate contact with the AMPA receptor.	bind
42642	1	9995	7	11	NULL	NULL	NULL	PICK1 dimer	GP		bind					PKC receptor subunit	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_6_919_s_131	10727702	A dimer of PICK1 could bind to both PKC  and AMPA receptor subunits, bringing active PKC  into intimate contact with the AMPA receptor.	bind
42643	2	9995	7	11	NULL	NULL	NULL	PICK1 dimer	GP		bind					AMPA receptor subunit	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_6_919_s_131	10727702	A dimer of PICK1 could bind to both PKC  and AMPA receptor subunits, bringing active PKC  into intimate contact with the AMPA receptor.	bind
42644	3	9995	7	11	NULL	NULL	NULL	PKC	GP	active	contact with		intimate			AMPA receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_6_919_s_131	10727702	A dimer of PICK1 could bind to both PKC  and AMPA receptor subunits, bringing active PKC  into intimate contact with the AMPA receptor.	bind
42645	4	9995	7	11	NULL	NULL	NULL	statement 1	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_6_919_s_131	10727702	A dimer of PICK1 could bind to both PKC  and AMPA receptor subunits, bringing active PKC  into intimate contact with the AMPA receptor.	bind
42646	5	9995	7	11	NULL	NULL	NULL	statement 2	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_6_919_s_131	10727702	A dimer of PICK1 could bind to both PKC  and AMPA receptor subunits, bringing active PKC  into intimate contact with the AMPA receptor.	bind
34851	1	9996	6	11	NULL	NULL	NULL	SRF dimer	GP		bind									SRE at 300 in promoter	NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_21_12202_s_38	9770464	A dimer of SRF and one molecule of Elk-1 (also known as TCF, ternary complex factor) bind to the serum response element (SRE) centered at  300 in the promoter ( 27).	bind
34852	2	9996	6	11	NULL	NULL	NULL	Elk-1	GP		is a synonym of					TCF	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_21_12202_s_38	9770464	A dimer of SRF and one molecule of Elk-1 (also known as TCF, ternary complex factor) bind to the serum response element (SRE) centered at  300 in the promoter ( 27).	bind
34853	3	9996	6	11	NULL	NULL	NULL	TCF	GP		is					ternary complex factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_21_12202_s_38	9770464	A dimer of SRF and one molecule of Elk-1 (also known as TCF, ternary complex factor) bind to the serum response element (SRE) centered at  300 in the promoter ( 27).	bind
34854	4	9996	6	11	NULL	NULL	NULL	Elk-1	GP		bind									SRE at 300 in promoter	NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_21_12202_s_38	9770464	A dimer of SRF and one molecule of Elk-1 (also known as TCF, ternary complex factor) bind to the serum response element (SRE) centered at  300 in the promoter ( 27).	bind
34855	5	9996	6	11	NULL	NULL	NULL	SRE	GP		is					serum response element	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_21_12202_s_38	9770464	A dimer of SRF and one molecule of Elk-1 (also known as TCF, ternary complex factor) bind to the serum response element (SRE) centered at  300 in the promoter ( 27).	bind
42647	1	9996	7	11	NULL	NULL	NULL	SRF dimer	GP		bind									SRE at 300 in the promoter	NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_21_12202_s_38	9770464	A dimer of SRF and one molecule of Elk-1 (also known as TCF, ternary complex factor) bind to the serum response element (SRE) centered at  300 in the promoter ( 27).	bind
42648	2	9996	7	11	NULL	NULL	NULL	Elk-1 	GP		bind									SRE at 300 in the promoter	NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_21_12202_s_38	9770464	A dimer of SRF and one molecule of Elk-1 (also known as TCF, ternary complex factor) bind to the serum response element (SRE) centered at  300 in the promoter ( 27).	bind
42649	3	9996	7	11	NULL	NULL	NULL	Elk-1 	GP		is a synonym of					TCF	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_21_12202_s_38	9770464	A dimer of SRF and one molecule of Elk-1 (also known as TCF, ternary complex factor) bind to the serum response element (SRE) centered at  300 in the promoter ( 27).	bind
42650	4	9996	7	11	NULL	NULL	NULL	TCF	GP		is					ternary complex factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_21_12202_s_38	9770464	A dimer of SRF and one molecule of Elk-1 (also known as TCF, ternary complex factor) bind to the serum response element (SRE) centered at  300 in the promoter ( 27).	bind
42651	5	9996	7	11	NULL	NULL	NULL	SRE	GP		is					serum response element	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_21_12202_s_38	9770464	A dimer of SRF and one molecule of Elk-1 (also known as TCF, ternary complex factor) bind to the serum response element (SRE) centered at  300 in the promoter ( 27).	bind
34996	1	9997	6	11	NULL	NULL	NULL	IscA	GP		is a type of					FeS cluster biosynthesis protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_22_0_457_s_1112	16824008	A dimer of the FeS cluster biosynthesis protein IscA from cyanobacteria  binds a [2Fe2] cluster between two protomers and transfers it to [2Fe2] and [4Fe4]  apo proteins.	bind
34997	2	9997	6	11	NULL	NULL	NULL	IscA dimer	GP	cyanobacteria	bind					[2Fe2] cluster 	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_22_0_457_s_1112	16824008	A dimer of the FeS cluster biosynthesis protein IscA from cyanobacteria  binds a [2Fe2] cluster between two protomers and transfers it to [2Fe2] and [4Fe4]  apo proteins.	bind
34998	3	9997	6	11	NULL	NULL	NULL	[2Fe2] cluster 	Chemical		is transfered to					[2Fe2] apo protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_22_0_457_s_1112	16824008	A dimer of the FeS cluster biosynthesis protein IscA from cyanobacteria  binds a [2Fe2] cluster between two protomers and transfers it to [2Fe2] and [4Fe4]  apo proteins.	bind
34999	4	9997	6	11	NULL	NULL	NULL	[2Fe2] cluster	Chemical		is transfered to					[4Fe4] apo protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_22_0_457_s_1112	16824008	A dimer of the FeS cluster biosynthesis protein IscA from cyanobacteria  binds a [2Fe2] cluster between two protomers and transfers it to [2Fe2] and [4Fe4]  apo proteins.	bind
35000	5	9997	6	11	NULL	NULL	NULL	statement 3	Process		occurs simultaneously with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_22_0_457_s_1112	16824008	A dimer of the FeS cluster biosynthesis protein IscA from cyanobacteria  binds a [2Fe2] cluster between two protomers and transfers it to [2Fe2] and [4Fe4]  apo proteins.	bind
35001	6	9997	6	11	NULL	NULL	NULL	statement 2	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_22_0_457_s_1112	16824008	A dimer of the FeS cluster biosynthesis protein IscA from cyanobacteria  binds a [2Fe2] cluster between two protomers and transfers it to [2Fe2] and [4Fe4]  apo proteins.	bind
35002	7	9997	6	11	NULL	NULL	NULL	statement 2	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_22_0_457_s_1112	16824008	A dimer of the FeS cluster biosynthesis protein IscA from cyanobacteria  binds a [2Fe2] cluster between two protomers and transfers it to [2Fe2] and [4Fe4]  apo proteins.	bind
42652	1	9997	7	11	NULL	NULL	NULL	IscA dimer	GP	cyanobacteria	binds					[2Fe2] cluster	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_22_0_457_s_1112	16824008	A dimer of the FeS cluster biosynthesis protein IscA from cyanobacteria  binds a [2Fe2] cluster between two protomers and transfers it to [2Fe2] and [4Fe4]  apo proteins.	bind
42653	2	9997	7	11	NULL	NULL	NULL	[2Fe2] cluster 	Chemical		is transfered to					[2Fe2] apo protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_22_0_457_s_1112	16824008	A dimer of the FeS cluster biosynthesis protein IscA from cyanobacteria  binds a [2Fe2] cluster between two protomers and transfers it to [2Fe2] and [4Fe4]  apo proteins.	bind
42654	3	9997	7	11	NULL	NULL	NULL	[2Fe2] cluster	Chemical		is transfered to					[4Fe4] apo protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_22_0_457_s_1112	16824008	A dimer of the FeS cluster biosynthesis protein IscA from cyanobacteria  binds a [2Fe2] cluster between two protomers and transfers it to [2Fe2] and [4Fe4]  apo proteins.	bind
42655	4	9997	7	11	NULL	NULL	NULL	IscA	GP		is a type of					FeS cluster biosynthesis protein 	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_22_0_457_s_1112	16824008	A dimer of the FeS cluster biosynthesis protein IscA from cyanobacteria  binds a [2Fe2] cluster between two protomers and transfers it to [2Fe2] and [4Fe4]  apo proteins.	bind
49149	5	9997	7	11	NULL	NULL	NULL	statement 2	Process		occurs simultaneously with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_22_0_457_s_1112	16824008	A dimer of the FeS cluster biosynthesis protein IscA from cyanobacteria  binds a [2Fe2] cluster between two protomers and transfers it to [2Fe2] and [4Fe4]  apo proteins.	bind
49150	6	9997	7	11	NULL	NULL	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_22_0_457_s_1112	16824008	A dimer of the FeS cluster biosynthesis protein IscA from cyanobacteria  binds a [2Fe2] cluster between two protomers and transfers it to [2Fe2] and [4Fe4]  apo proteins.	bind
49151	7	9997	7	11	NULL	NULL	NULL	statement 1	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_22_0_457_s_1112	16824008	A dimer of the FeS cluster biosynthesis protein IscA from cyanobacteria  binds a [2Fe2] cluster between two protomers and transfers it to [2Fe2] and [4Fe4]  apo proteins.	bind
35003	1	10000	6	11	NULL	NULL	NULL	importin	GP		bind								NLS		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_2_89_s_20	9427645	A dimeric receptor comprising importin    (that binds the NLS) and importin    (that mediates translocation) imports proteins bearing the classical NLS motif, which contains basic residues      [1-4,15]  .	bind
35004	2	10000	6	11	NULL	NULL	NULL	importin	GP		mediates					translocation	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_2_89_s_20	9427645	A dimeric receptor comprising importin    (that binds the NLS) and importin    (that mediates translocation) imports proteins bearing the classical NLS motif, which contains basic residues      [1-4,15]  .	bind
35005	3	10000	6	11	NULL	NULL	NULL	dimeric receptor	GP		comprise					statement 1 & statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_2_89_s_20	9427645	A dimeric receptor comprising importin    (that binds the NLS) and importin    (that mediates translocation) imports proteins bearing the classical NLS motif, which contains basic residues      [1-4,15]  .	bind
35006	4	10000	6	11	NULL	NULL	NULL	statement 3	Process		imports 					proteins 	GP		classical NLS motif		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_2_89_s_20	9427645	A dimeric receptor comprising importin    (that binds the NLS) and importin    (that mediates translocation) imports proteins bearing the classical NLS motif, which contains basic residues      [1-4,15]  .	bind
35007	5	10000	6	11	NULL	NULL	NULL				contains			classical NLS motif		basic residues	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_2_89_s_20	9427645	A dimeric receptor comprising importin    (that binds the NLS) and importin    (that mediates translocation) imports proteins bearing the classical NLS motif, which contains basic residues      [1-4,15]  .	bind
42656	3	10000	7	11	NULL	NULL	NULL	dimeric receptor	GP		comprise					statement 1 & statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_2_89_s_20	9427645	A dimeric receptor comprising importin    (that binds the NLS) and importin    (that mediates translocation) imports proteins bearing the classical NLS motif, which contains basic residues      [1-4,15]  .	bind
42657	1	10000	7	11	NULL	NULL	NULL	importin	GP		binds								NLS		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_2_89_s_20	9427645	A dimeric receptor comprising importin    (that binds the NLS) and importin    (that mediates translocation) imports proteins bearing the classical NLS motif, which contains basic residues      [1-4,15]  .	bind
42658	2	10000	7	11	NULL	NULL	NULL	importin	GP		mediates					translocation	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_2_89_s_20	9427645	A dimeric receptor comprising importin    (that binds the NLS) and importin    (that mediates translocation) imports proteins bearing the classical NLS motif, which contains basic residues      [1-4,15]  .	bind
42660	4	10000	7	11	NULL	NULL	NULL	statement 3	Process		imports					proteins	GP		 classical NLS motif		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_2_89_s_20	9427645	A dimeric receptor comprising importin    (that binds the NLS) and importin    (that mediates translocation) imports proteins bearing the classical NLS motif, which contains basic residues      [1-4,15]  .	bind
42661	5	10000	7	11	NULL	NULL	NULL				contains			classical NLS motif		basic residues	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_2_89_s_20	9427645	A dimeric receptor comprising importin    (that binds the NLS) and importin    (that mediates translocation) imports proteins bearing the classical NLS motif, which contains basic residues      [1-4,15]  .	bind
35008	1	10001	6	11	NULL	NULL	NULL	p85	GP		bind					IRS-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_11_2569_s_169	8647950	A diminished binding of p85 to IRS-1 containing the Gly  Arg  substitution could be due to an effect of the mutation on the  tertiary structure of IRS-1.	bind
35009	2	10001	6	11	NULL	NULL	NULL	IRS-1	GP		effects			Gly Arg substitution		IRS-1	GP	tertiary structure of			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_11_2569_s_169	8647950	A diminished binding of p85 to IRS-1 containing the Gly  Arg  substitution could be due to an effect of the mutation on the  tertiary structure of IRS-1.	bind
35010	3	10001	6	11	NULL	NULL	NULL	p85	GP		bind					IRS-1	GP		Gly Arg substitution		NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_11_2569_s_169	8647950	A diminished binding of p85 to IRS-1 containing the Gly  Arg  substitution could be due to an effect of the mutation on the  tertiary structure of IRS-1.	bind
35011	4	10001	6	11	NULL	NULL	NULL	statement 1	Process	affinity of	is less than					statement 3	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_11_2569_s_169	8647950	A diminished binding of p85 to IRS-1 containing the Gly  Arg  substitution could be due to an effect of the mutation on the  tertiary structure of IRS-1.	bind
35012	5	10001	6	11	NULL	NULL	NULL	statement 4	Process		could be due to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_11_2569_s_169	8647950	A diminished binding of p85 to IRS-1 containing the Gly  Arg  substitution could be due to an effect of the mutation on the  tertiary structure of IRS-1.	bind
42662	1	10001	7	11	NULL	NULL	NULL	IRS-1	GP		substituted with			Gly		IRS-1	GP		Arg		NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_11_2569_s_169	8647950	A diminished binding of p85 to IRS-1 containing the Gly  Arg  substitution could be due to an effect of the mutation on the  tertiary structure of IRS-1.	bind
42663	2	10001	7	11	NULL	NULL	NULL	p85	GP		bind					IRS-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_11_2569_s_169	8647950	A diminished binding of p85 to IRS-1 containing the Gly  Arg  substitution could be due to an effect of the mutation on the  tertiary structure of IRS-1.	bind
57614	3	10001	7	11	NULL	NULL	NULL	p85	GP		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_11_2569_s_169	8647950	A diminished binding of p85 to IRS-1 containing the Gly  Arg  substitution could be due to an effect of the mutation on the  tertiary structure of IRS-1.	bind
57615	4	10001	7	11	NULL	NULL	NULL	statement 3	Process	affinity of	is lesser than					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_11_2569_s_169	8647950	A diminished binding of p85 to IRS-1 containing the Gly  Arg  substitution could be due to an effect of the mutation on the  tertiary structure of IRS-1.	bind
57616	5	10001	7	11	NULL	NULL	NULL	mutation	Process		effect					IRS-1	GP	tertiary structure of			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_11_2569_s_169	8647950	A diminished binding of p85 to IRS-1 containing the Gly  Arg  substitution could be due to an effect of the mutation on the  tertiary structure of IRS-1.	bind
57617	6	10001	7	11	NULL	NULL	NULL	statement 4	Process		because of					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_11_2569_s_169	8647950	A diminished binding of p85 to IRS-1 containing the Gly  Arg  substitution could be due to an effect of the mutation on the  tertiary structure of IRS-1.	bind
35013	1	10002	6	11	NULL	NULL	NULL	UBR1	GP		bind					N-degron	AminoAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7120_s_256	16055722	A dipeptide bearing type 1 or type 2 N-degron competitively inhibits the in vitro binding of UBR1 and UBR2 to N-degron ( ,  ).	bind
35014	2	10002	6	11	NULL	NULL	NULL	UBR2	GP		bind					N-degron	AminoAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7120_s_256	16055722	A dipeptide bearing type 1 or type 2 N-degron competitively inhibits the in vitro binding of UBR1 and UBR2 to N-degron ( ,  ).	bind
35015	3	10002	6	11	NULL	NULL	NULL	dipeptide bearing type 1 N-degron	AminoAcid		inhibits		competitively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7120_s_256	16055722	A dipeptide bearing type 1 or type 2 N-degron competitively inhibits the in vitro binding of UBR1 and UBR2 to N-degron ( ,  ).	bind
35016	4	10002	6	11	NULL	NULL	NULL	dipeptide bearing type 1 N-degron	AminoAcid		inhibits		competitively			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7120_s_256	16055722	A dipeptide bearing type 1 or type 2 N-degron competitively inhibits the in vitro binding of UBR1 and UBR2 to N-degron ( ,  ).	bind
35017	5	10002	6	11	NULL	NULL	NULL	dipeptide bearing type 2 N-degron	AminoAcid		inhibits		competitively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7120_s_256	16055722	A dipeptide bearing type 1 or type 2 N-degron competitively inhibits the in vitro binding of UBR1 and UBR2 to N-degron ( ,  ).	bind
35018	6	10002	6	11	NULL	NULL	NULL	dipeptide bearing type 2 N-degron	AminoAcid		inhibits		competitively			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7120_s_256	16055722	A dipeptide bearing type 1 or type 2 N-degron competitively inhibits the in vitro binding of UBR1 and UBR2 to N-degron ( ,  ).	bind
35019	7	10002	6	11	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7120_s_256	16055722	A dipeptide bearing type 1 or type 2 N-degron competitively inhibits the in vitro binding of UBR1 and UBR2 to N-degron ( ,  ).	bind
35020	8	10002	6	11	NULL	NULL	NULL	statement 4	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7120_s_256	16055722	A dipeptide bearing type 1 or type 2 N-degron competitively inhibits the in vitro binding of UBR1 and UBR2 to N-degron ( ,  ).	bind
42664	1	10002	7	11	NULL	NULL	NULL	 UBR1	GP		bind					N-degron	AminoAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7120_s_256	16055722	A dipeptide bearing type 1 or type 2 N-degron competitively inhibits the in vitro binding of UBR1 and UBR2 to N-degron ( ,  ).	bind
42665	2	10002	7	11	NULL	NULL	NULL	UBR2	GP		bind					N-degron	AminoAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7120_s_256	16055722	A dipeptide bearing type 1 or type 2 N-degron competitively inhibits the in vitro binding of UBR1 and UBR2 to N-degron ( ,  ).	bind
42666	3	10002	7	11	NULL	NULL	NULL	dipeptide bearing type 1 N-degron 	AminoAcid		inhibits		competitively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7120_s_256	16055722	A dipeptide bearing type 1 or type 2 N-degron competitively inhibits the in vitro binding of UBR1 and UBR2 to N-degron ( ,  ).	bind
42667	4	10002	7	11	NULL	NULL	NULL	dipeptide bearing type 1 N-degron 	AminoAcid		inhibits		competitively			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7120_s_256	16055722	A dipeptide bearing type 1 or type 2 N-degron competitively inhibits the in vitro binding of UBR1 and UBR2 to N-degron ( ,  ).	bind
42668	5	10002	7	11	NULL	NULL	NULL	dipeptide bearing type 2 N-degron 	AminoAcid		inhibits		competitively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7120_s_256	16055722	A dipeptide bearing type 1 or type 2 N-degron competitively inhibits the in vitro binding of UBR1 and UBR2 to N-degron ( ,  ).	bind
42669	6	10002	7	11	NULL	NULL	NULL	dipeptide bearing type 2 N-degron 	AminoAcid		inhibits		competitively			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7120_s_256	16055722	A dipeptide bearing type 1 or type 2 N-degron competitively inhibits the in vitro binding of UBR1 and UBR2 to N-degron ( ,  ).	bind
49152	7	10002	7	11	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7120_s_256	16055722	A dipeptide bearing type 1 or type 2 N-degron competitively inhibits the in vitro binding of UBR1 and UBR2 to N-degron ( ,  ).	bind
49153	8	10002	7	11	NULL	NULL	NULL	statement 4	Process		is an alternative to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_16_7120_s_256	16055722	A dipeptide bearing type 1 or type 2 N-degron competitively inhibits the in vitro binding of UBR1 and UBR2 to N-degron ( ,  ).	bind
35074	1	10003	6	11	NULL	NULL	NULL	DP IV	GP		is a type of					aminopeptidase	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_9_5063_s_8	12690074	A dipeptide mimicking inhibitor complexed to the active site discloses key determinants for substrate recognition, including a Glu-Glu motif that distinguishes DP IV as an aminopeptidase and an oxyanion trap that binds and activates the P2-carbonyl oxygen necessary for efficient postproline cleavage.	bind
35075	2	10003	6	11	NULL	NULL	NULL	oxyanion trap	Chemical		bind					P2-carbonyl oxygen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_9_5063_s_8	12690074	A dipeptide mimicking inhibitor complexed to the active site discloses key determinants for substrate recognition, including a Glu-Glu motif that distinguishes DP IV as an aminopeptidase and an oxyanion trap that binds and activates the P2-carbonyl oxygen necessary for efficient postproline cleavage.	bind
35076	3	10003	6	11	NULL	NULL	NULL	statement 2	Process		activates					P2-carbonyl oxygen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_9_5063_s_8	12690074	A dipeptide mimicking inhibitor complexed to the active site discloses key determinants for substrate recognition, including a Glu-Glu motif that distinguishes DP IV as an aminopeptidase and an oxyanion trap that binds and activates the P2-carbonyl oxygen necessary for efficient postproline cleavage.	bind
35077	4	10003	6	11	NULL	NULL	NULL	statement 3	Process		is necessary for					postproline	AminoAcid	efficient cleavage of 			NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_9_5063_s_8	12690074	A dipeptide mimicking inhibitor complexed to the active site discloses key determinants for substrate recognition, including a Glu-Glu motif that distinguishes DP IV as an aminopeptidase and an oxyanion trap that binds and activates the P2-carbonyl oxygen necessary for efficient postproline cleavage.	bind
42678	1	10003	7	11	NULL	NULL	NULL	oxyanion trap	Chemical		binds					P2-carbonyl oxygen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_9_5063_s_8	12690074	A dipeptide mimicking inhibitor complexed to the active site discloses key determinants for substrate recognition, including a Glu-Glu motif that distinguishes DP IV as an aminopeptidase and an oxyanion trap that binds and activates the P2-carbonyl oxygen necessary for efficient postproline cleavage.	bind
42679	2	10003	7	11	NULL	NULL	NULL	statement 1	Process		activates					P2-carbonyl oxygen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_9_5063_s_8	12690074	A dipeptide mimicking inhibitor complexed to the active site discloses key determinants for substrate recognition, including a Glu-Glu motif that distinguishes DP IV as an aminopeptidase and an oxyanion trap that binds and activates the P2-carbonyl oxygen necessary for efficient postproline cleavage.	bind
42680	3	10003	7	11	NULL	NULL	NULL	statement 2	Process		is necessary for					postproline	AminoAcid	efficient cleavage of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_9_5063_s_8	12690074	A dipeptide mimicking inhibitor complexed to the active site discloses key determinants for substrate recognition, including a Glu-Glu motif that distinguishes DP IV as an aminopeptidase and an oxyanion trap that binds and activates the P2-carbonyl oxygen necessary for efficient postproline cleavage.	bind
42685	4	10003	7	11	NULL	NULL	NULL	DP IV	GP		is a type of					aminopeptidase	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_9_5063_s_8	12690074	A dipeptide mimicking inhibitor complexed to the active site discloses key determinants for substrate recognition, including a Glu-Glu motif that distinguishes DP IV as an aminopeptidase and an oxyanion trap that binds and activates the P2-carbonyl oxygen necessary for efficient postproline cleavage.	bind
35023	1	10005	6	11	NULL	NULL	NULL	She2p	GP		bind		directly			She3p	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_19_20_5514_s_247	11032818	A direct  ASH1 RNA-independent binding of She2p and She3p is suggested by our  in vitro pulldown experiments.	bind
35024	2	10005	6	11	NULL	NULL	NULL	statement 1	Process		is independent of					ASH1 RNA	NucleicAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_19_20_5514_s_247	11032818	A direct  ASH1 RNA-independent binding of She2p and She3p is suggested by our  in vitro pulldown experiments.	bind
42721	1	10005	7	11	NULL	NULL	NULL	She2p	GP		bind		directly			She3p	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_19_20_5514_s_247	11032818	A direct  ASH1 RNA-independent binding of She2p and She3p is suggested by our  in vitro pulldown experiments.	bind
42722	2	10005	7	11	NULL	NULL	NULL	statement 1	Process		is independent of					ASH1 RNA	NucleicAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_19_20_5514_s_247	11032818	A direct  ASH1 RNA-independent binding of She2p and She3p is suggested by our  in vitro pulldown experiments.	bind
35025	1	10006	6	11	NULL	NULL	NULL	DAG	Chemical	PC-derived	activates		directly			Raf-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_36_21299_s_17	7673165	A direct activation of  Raf-1 by PC-derived DAG may also be possible since the enzyme contains  a cysteine finger in the regulatory domain similar to the DAG binding  motifs of PKC and DAG kinase( 20) .	bind
35026	2	10006	6	11	NULL	NULL	NULL	DAG	Chemical	PC-derived	is similar to			cysteine finger in the regulatory domain		PKC kinase	GP		DAG binding motif		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_36_21299_s_17	7673165	A direct activation of  Raf-1 by PC-derived DAG may also be possible since the enzyme contains  a cysteine finger in the regulatory domain similar to the DAG binding  motifs of PKC and DAG kinase( 20) .	bind
35027	3	10006	6	11	NULL	NULL	NULL	DAG	Chemical	PC-derived	is similar to			cysteine finger in the regulatory domain		DAG kinase	GP		DAG binding motif		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_36_21299_s_17	7673165	A direct activation of  Raf-1 by PC-derived DAG may also be possible since the enzyme contains  a cysteine finger in the regulatory domain similar to the DAG binding  motifs of PKC and DAG kinase( 20) .	bind
35029	4	10006	6	11	NULL	NULL	NULL	statement 1	Process		occurs due to		may			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_36_21299_s_17	7673165	A direct activation of  Raf-1 by PC-derived DAG may also be possible since the enzyme contains  a cysteine finger in the regulatory domain similar to the DAG binding  motifs of PKC and DAG kinase( 20) .	bind
35030	5	10006	6	11	NULL	NULL	NULL	statement 1	Process		occurs due to		may			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_36_21299_s_17	7673165	A direct activation of  Raf-1 by PC-derived DAG may also be possible since the enzyme contains  a cysteine finger in the regulatory domain similar to the DAG binding  motifs of PKC and DAG kinase( 20) .	bind
42725	1	10006	7	11	NULL	NULL	NULL	DAG 	Chemical	PC-derived	activates		directly			Raf-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_36_21299_s_17	7673165	A direct activation of  Raf-1 by PC-derived DAG may also be possible since the enzyme contains  a cysteine finger in the regulatory domain similar to the DAG binding  motifs of PKC and DAG kinase( 20) .	bind
42726	2	10006	7	11	NULL	NULL	NULL	 DAG 	Chemical	PC-derived	is similar to			cysteine finger in the regulatory domain		PKC kinase	GP		DAG binding motif		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_36_21299_s_17	7673165	A direct activation of  Raf-1 by PC-derived DAG may also be possible since the enzyme contains  a cysteine finger in the regulatory domain similar to the DAG binding  motifs of PKC and DAG kinase( 20) .	bind
42727	3	10006	7	11	NULL	NULL	NULL	DAG	Chemical	PC-derived	is similar to			cysteine finger in the regulatory domain		DAG kinase	GP		DAG binding motifs		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_36_21299_s_17	7673165	A direct activation of  Raf-1 by PC-derived DAG may also be possible since the enzyme contains  a cysteine finger in the regulatory domain similar to the DAG binding  motifs of PKC and DAG kinase( 20) .	bind
42728	4	10006	7	11	NULL	NULL	NULL	statement 1	Process		occurs due to		may			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_36_21299_s_17	7673165	A direct activation of  Raf-1 by PC-derived DAG may also be possible since the enzyme contains  a cysteine finger in the regulatory domain similar to the DAG binding  motifs of PKC and DAG kinase( 20) .	bind
49330	5	10006	7	11	NULL	NULL	NULL	statement 1	Process		occurs due to		may			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_36_21299_s_17	7673165	A direct activation of  Raf-1 by PC-derived DAG may also be possible since the enzyme contains  a cysteine finger in the regulatory domain similar to the DAG binding  motifs of PKC and DAG kinase( 20) .	bind
49556	1	10007	6	11	NULL	NULL	NULL			mutant	effects			Gly-294		L-serine	AminoAcid	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_21_17844_s_104	11278587	A direct analysis of L-serine binding by equilibrium dialysis was performed to look at the effect of mutating Gly-294 on serine binding (Fig.  5).	bind
42729	1	10007	7	11	NULL	NULL	NULL			mutant	effect			Gly-294		L-serine	AminoAcid	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_21_17844_s_104	11278587	A direct analysis of L-serine binding by equilibrium dialysis was performed to look at the effect of mutating Gly-294 on serine binding (Fig.  5).	bind
49561	1	10008	6	11	NULL	NULL	NULL	vitronectin	GP		bind					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1545_1_289_s_131	11342054	A direct assay was used to measure vitronectin binding to heparin-coated microtiter plates.	bind
42730	1	10008	7	11	NULL	NULL	NULL	vitronectin	GP		bind					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1545_1_289_s_131	11342054	A direct assay was used to measure vitronectin binding to heparin-coated microtiter plates.	bind
35031	1	10009	6	11	NULL	NULL	NULL	DEDD	GP	FLAG-tagged;; in vitro translated	bind					ubiquitin	GP				NULL		NULL	NULL	NULL	NULL	gw70_amjpathol_164_2_395_s_168	14742246	A direct binding assay of FLAG-tagged,  in vitro translated, DEDD shows binding of DEDD, but not the dominant-negative derivative  of FADD (DN-FADD), to ubiquitin Sepharose (Ubi-Seph).	bind
35032	2	10009	6	11	NULL	NULL	NULL	DN-FADD	GP		does not bind					ubiquitin	GP				NULL		NULL	NULL	NULL	NULL	gw70_amjpathol_164_2_395_s_168	14742246	A direct binding assay of FLAG-tagged,  in vitro translated, DEDD shows binding of DEDD, but not the dominant-negative derivative  of FADD (DN-FADD), to ubiquitin Sepharose (Ubi-Seph).	bind
35033	3	10009	6	11	NULL	NULL	NULL	DN-FADD	GP		is					dominant-negative derivative of FADD	GP				NULL		NULL	NULL	NULL	NULL	gw70_amjpathol_164_2_395_s_168	14742246	A direct binding assay of FLAG-tagged,  in vitro translated, DEDD shows binding of DEDD, but not the dominant-negative derivative  of FADD (DN-FADD), to ubiquitin Sepharose (Ubi-Seph).	bind
42731	1	10009	7	11	NULL	NULL	NULL	DEDD	GP	FLAG-tagged;;in vitro translated	bind					ubiquitin	GP				NULL		NULL	NULL	NULL	NULL	gw70_amjpathol_164_2_395_s_168	14742246	A direct binding assay of FLAG-tagged,  in vitro translated, DEDD shows binding of DEDD, but not the dominant-negative derivative  of FADD (DN-FADD), to ubiquitin Sepharose (Ubi-Seph).	bind
42732	2	10009	7	11	NULL	NULL	NULL	DN-FADD	GP		does not bind					ubiquitin	GP				NULL		NULL	NULL	NULL	NULL	gw70_amjpathol_164_2_395_s_168	14742246	A direct binding assay of FLAG-tagged,  in vitro translated, DEDD shows binding of DEDD, but not the dominant-negative derivative  of FADD (DN-FADD), to ubiquitin Sepharose (Ubi-Seph).	bind
42733	3	10009	7	11	NULL	NULL	NULL	DN-FADD	GP		is					dominant-negative derivative of FADD 	GP				NULL		NULL	NULL	NULL	NULL	gw70_amjpathol_164_2_395_s_168	14742246	A direct binding assay of FLAG-tagged,  in vitro translated, DEDD shows binding of DEDD, but not the dominant-negative derivative  of FADD (DN-FADD), to ubiquitin Sepharose (Ubi-Seph).	bind
57238	1	10010	6	10	NULL	0	NULL	Rdr1p			does not bind		directly			PDR5					NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_70_3_583_s_419	16959962	A direct binding of Rdr1p to  PDR5 has not been demonstrated, and the mode of binding (e.g., monomer or heterodimer)  of Yrm1p (in orange) is not known.	bind
42735	1	10010	7	NULL	NULL	0	NULL	Rdr1p	NULL		does not bind	NULL	directly			PDR5	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_70_3_583_s_419	16959962	A direct binding of Rdr1p to  PDR5 has not been demonstrated, and the mode of binding (e.g., monomer or heterodimer)  of Yrm1p (in orange) is not known.	bind
35034	1	10011	6	11	NULL	NULL	NULL	125I-FX	GP		bind		directly			sTF	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_5_3622_s_405	11723140	A direct binding plot for binding of 125I-FX to sTF is presented in Fig.  9 A and the  K d(app) obtained from this plot for binding of FX to sTF was 500  plus-or-minus  100 nM.	bind
42736	1	10011	7	11	NULL	NULL	NULL	125I-FX	GP		bind		directly			sTF	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_5_3622_s_405	11723140	A direct binding plot for binding of 125I-FX to sTF is presented in Fig.  9 A and the  K d(app) obtained from this plot for binding of FX to sTF was 500  plus-or-minus  100 nM.	bind
35035	1	10012	6	11	NULL	NULL	NULL	Phab B7	GP		has affinity for		high			B7 clone	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_19_5571_s_194	11544219	A direct comparison by ELISA of the binding properties of Phab B7 and Phab B9 also revealed a higher affinity of the B7 clone (Fig.  3).	bind
35036	2	10012	6	11	NULL	NULL	NULL	Phab B9	GP		has affinity for		high			B7 clone	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_19_5571_s_194	11544219	A direct comparison by ELISA of the binding properties of Phab B7 and Phab B9 also revealed a higher affinity of the B7 clone (Fig.  3).	bind
42737	1	10012	7	11	NULL	NULL	NULL	B7 clone	GP		affinity for		high			Phab B7	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_19_5571_s_194	11544219	A direct comparison by ELISA of the binding properties of Phab B7 and Phab B9 also revealed a higher affinity of the B7 clone (Fig.  3).	bind
42738	2	10012	7	11	NULL	NULL	NULL	B7 clone	GP		affinity for		high			Phab B9	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_19_5571_s_194	11544219	A direct comparison by ELISA of the binding properties of Phab B7 and Phab B9 also revealed a higher affinity of the B7 clone (Fig.  3).	bind
35037	1	10013	6	11	NULL	NULL	NULL	FKBP12	GP		bind		may			RyR	GP	cardiac			NULL	intact cells	NULL	NULL	NULL	NULL	gw60_circulationres_88_2_134_s_38	11157663	A direct comparison of control and FKBP12.6-overexpressing cells was therefore valid, because although in vitro experiments indicate that cardiac RyRs are poor substrates for FKBP12, 14 15  binding of FKBP12 to cardiac RyRs in intact cells has not been ruled out.	bind
35038	2	10013	6	3	NULL	0	NULL	RyR	GP	cardiac	substrate for		poor			FKBP12	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulationres_88_2_134_s_38	11157663	A direct comparison of control and FKBP12.6-overexpressing cells was therefore valid, because although in vitro experiments indicate that cardiac RyRs are poor substrates for FKBP12, 14 15  binding of FKBP12 to cardiac RyRs in intact cells has not been ruled out.	bind
42739	1	10013	7	3	NULL	0	NULL	RyRs	GP	cardiac	substrate for		poor			FKBP12	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_circulationres_88_2_134_s_38	11157663	A direct comparison of control and FKBP12.6-overexpressing cells was therefore valid, because although in vitro experiments indicate that cardiac RyRs are poor substrates for FKBP12, 14 15  binding of FKBP12 to cardiac RyRs in intact cells has not been ruled out.	bind
42742	4	10013	7	3	NULL	0	NULL	FKBP12	GP		bind		may			RyRs	GP	cardiac			NULL	intact cells	NULL	NULL	NULL	NULL	gw60_circulationres_88_2_134_s_38	11157663	A direct comparison of control and FKBP12.6-overexpressing cells was therefore valid, because although in vitro experiments indicate that cardiac RyRs are poor substrates for FKBP12, 14 15  binding of FKBP12 to cardiac RyRs in intact cells has not been ruled out.	bind
35039	1	10014	6	3	NULL	0	NULL	PLD	GP		bind					PC vesicles	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_50_35367_s_189	10585404	A direct comparison of PLD binding to PC and PS vesicles in the absence or presence of Ba2+ emphasizes this behavior	bind
35040	2	10014	6	3	NULL	0	NULL	PLD	GP		bind					PS vesicles	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_50_35367_s_189	10585404	A direct comparison of PLD binding to PC and PS vesicles in the absence or presence of Ba2+ emphasizes this behavior	bind
42743	1	10014	7	3	NULL	0	NULL	 PLD	GP		bind					PC vesicles	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_50_35367_s_189	10585404	A direct comparison of PLD binding to PC and PS vesicles in the absence or presence of Ba2+ emphasizes this behavior	bind
42744	2	10014	7	3	NULL	0	NULL	PLD	GP		bind					PS vesicles	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_50_35367_s_189	10585404	A direct comparison of PLD binding to PC and PS vesicles in the absence or presence of Ba2+ emphasizes this behavior	bind
35041	1	10015	6	3	NULL	0	NULL	ATP	Chemical		bind					Kir6.2	GP		C terminus		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_19_19097_s_173	15760904	A direct competition for binding between ATP and PIP2 at the C terminus of Kir6.2 has been reported ( ).	bind
35042	2	10015	6	3	NULL	0	NULL	PIP2	Chemical		bind					Kir6.2	GP		C terminus		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_19_19097_s_173	15760904	A direct competition for binding between ATP and PIP2 at the C terminus of Kir6.2 has been reported ( ).	bind
35043	3	10015	6	3	NULL	0	NULL	statement 1	Process		competes		directly			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_19_19097_s_173	15760904	A direct competition for binding between ATP and PIP2 at the C terminus of Kir6.2 has been reported ( ).	bind
42745	1	10015	7	3	NULL	0	NULL	ATP 	Chemical		bind					Kir6.2	GP		 C terminus		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_19_19097_s_173	15760904	A direct competition for binding between ATP and PIP2 at the C terminus of Kir6.2 has been reported ( ).	bind
42746	2	10015	7	3	NULL	0	NULL	PIP2	Chemical		bind					Kir6.2	GP		C terminus		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_19_19097_s_173	15760904	A direct competition for binding between ATP and PIP2 at the C terminus of Kir6.2 has been reported ( ).	bind
42747	3	10015	7	3	NULL	0	NULL	statement 1	Process		competes with		directly			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_19_19097_s_173	15760904	A direct competition for binding between ATP and PIP2 at the C terminus of Kir6.2 has been reported ( ).	bind
35044	1	10016	6	3	NULL	0	NULL	Vpu	GP		bind					beta-TrCP	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_280_5371_1880_s_89	9632380	A direct connection between Vpu and the proteasome was established by the demonstration that Vpu binds to a protein termed beta-TrCP, which in turn binds to the proteasome targeting factor Skp1p ( Fig. 3).	bind
35045	2	10016	6	3	NULL	0	NULL	statement 1	Process		bind					Skp1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_280_5371_1880_s_89	9632380	A direct connection between Vpu and the proteasome was established by the demonstration that Vpu binds to a protein termed beta-TrCP, which in turn binds to the proteasome targeting factor Skp1p ( Fig. 3).	bind
35046	3	10016	6	3	NULL	0	NULL	Skp1p	GP		is a type of					proteasome targeting factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_280_5371_1880_s_89	9632380	A direct connection between Vpu and the proteasome was established by the demonstration that Vpu binds to a protein termed beta-TrCP, which in turn binds to the proteasome targeting factor Skp1p ( Fig. 3).	bind
42748	1	10016	7	3	NULL	0	NULL	Vpu	GP		binds					beta-TrCP	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_280_5371_1880_s_89	9632380	A direct connection between Vpu and the proteasome was established by the demonstration that Vpu binds to a protein termed beta-TrCP, which in turn binds to the proteasome targeting factor Skp1p ( Fig. 3).	bind
42749	2	10016	7	3	NULL	0	NULL	statement 1	Process		binds					Skp1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_280_5371_1880_s_89	9632380	A direct connection between Vpu and the proteasome was established by the demonstration that Vpu binds to a protein termed beta-TrCP, which in turn binds to the proteasome targeting factor Skp1p ( Fig. 3).	bind
42750	3	10016	7	3	NULL	0	NULL	Skp1p	GP		is a type of					proteasome targeting factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_280_5371_1880_s_89	9632380	A direct connection between Vpu and the proteasome was established by the demonstration that Vpu binds to a protein termed beta-TrCP, which in turn binds to the proteasome targeting factor Skp1p ( Fig. 3).	bind
35047	1	10017	6	3	NULL	0	NULL	vitronectin	GP		bind					PAI-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_5112_s_197	9030577	A direct consequence of vitronectin binding to PAI-1 is that the half-life of the active conformation of the serpin is increased 2-3-fold ( 17-19).	bind
35048	2	10017	6	3	NULL	0	NULL	statement 1	Process		increases					serpin	GP	half life of;; active conformation of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_5112_s_197	9030577	A direct consequence of vitronectin binding to PAI-1 is that the half-life of the active conformation of the serpin is increased 2-3-fold ( 17-19).	bind
42751	1	10017	7	3	NULL	0	NULL	 vitronectin	GP		bind					PAI-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_5112_s_197	9030577	A direct consequence of vitronectin binding to PAI-1 is that the half-life of the active conformation of the serpin is increased 2-3-fold ( 17-19).	bind
42752	2	10017	7	3	NULL	0	NULL	statement 1	Process		increase					serpin	GP	half-life of;;active conformation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_5112_s_197	9030577	A direct consequence of vitronectin binding to PAI-1 is that the half-life of the active conformation of the serpin is increased 2-3-fold ( 17-19).	bind
35049	1	10018	6	11	NULL	NULL	NULL	PV IgG	GP		bind					KC	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29466_s_350	10899159	A direct evidence of activation of second messenger systems in response to PV IgG binding to KC have been obtained in the studies showing changes with phospholipase C, inositol 1,4,5-trisphosphate, transmembrane flux and intracellular levels of Ca2+, intracellular cAMP/cGMP ratios, and activity and intracellular location of protein kinase C (reviewed in Refs.	bind
35070	2	10018	6	11	NULL	NULL	NULL	Ca2+	Chemical		is a type of					second messenger	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29466_s_350	10899159	A direct evidence of activation of second messenger systems in response to PV IgG binding to KC have been obtained in the studies showing changes with phospholipase C, inositol 1,4,5-trisphosphate, transmembrane flux and intracellular levels of Ca2+, intracellular cAMP/cGMP ratios, and activity and intracellular location of protein kinase C (reviewed in Refs.	bind
35071	3	10018	6	11	NULL	NULL	NULL	cAMP/cGMP	Chemical		is a type of					second messenger	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29466_s_350	10899159	A direct evidence of activation of second messenger systems in response to PV IgG binding to KC have been obtained in the studies showing changes with phospholipase C, inositol 1,4,5-trisphosphate, transmembrane flux and intracellular levels of Ca2+, intracellular cAMP/cGMP ratios, and activity and intracellular location of protein kinase C (reviewed in Refs.	bind
35072	4	10018	6	11	NULL	NULL	NULL	Ca2+	Chemical	activation of	occurs in response to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29466_s_350	10899159	A direct evidence of activation of second messenger systems in response to PV IgG binding to KC have been obtained in the studies showing changes with phospholipase C, inositol 1,4,5-trisphosphate, transmembrane flux and intracellular levels of Ca2+, intracellular cAMP/cGMP ratios, and activity and intracellular location of protein kinase C (reviewed in Refs.	bind
35073	5	10018	6	11	NULL	NULL	NULL	cAMP/cGMP	Chemical	activation of	occurs in response to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29466_s_350	10899159	A direct evidence of activation of second messenger systems in response to PV IgG binding to KC have been obtained in the studies showing changes with phospholipase C, inositol 1,4,5-trisphosphate, transmembrane flux and intracellular levels of Ca2+, intracellular cAMP/cGMP ratios, and activity and intracellular location of protein kinase C (reviewed in Refs.	bind
42753	1	10018	7	11	NULL	NULL	NULL	PV IgG	GP		bind					KC	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29466_s_350	10899159	A direct evidence of activation of second messenger systems in response to PV IgG binding to KC have been obtained in the studies showing changes with phospholipase C, inositol 1,4,5-trisphosphate, transmembrane flux and intracellular levels of Ca2+, intracellular cAMP/cGMP ratios, and activity and intracellular location of protein kinase C (reviewed in Refs.	bind
42754	2	10018	7	11	NULL	NULL	NULL	statement 1	Process		activates					second messenger systems	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29466_s_350	10899159	A direct evidence of activation of second messenger systems in response to PV IgG binding to KC have been obtained in the studies showing changes with phospholipase C, inositol 1,4,5-trisphosphate, transmembrane flux and intracellular levels of Ca2+, intracellular cAMP/cGMP ratios, and activity and intracellular location of protein kinase C (reviewed in Refs.	bind
42755	3	10018	7	11	NULL	NULL	NULL	statement 1	GP		activates					phospholipase C	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29466_s_350	10899159	A direct evidence of activation of second messenger systems in response to PV IgG binding to KC have been obtained in the studies showing changes with phospholipase C, inositol 1,4,5-trisphosphate, transmembrane flux and intracellular levels of Ca2+, intracellular cAMP/cGMP ratios, and activity and intracellular location of protein kinase C (reviewed in Refs.	bind
42756	4	10018	7	11	NULL	NULL	NULL	statement 1	GP		activates					inositol 1,4,5-trisphosphate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29466_s_350	10899159	A direct evidence of activation of second messenger systems in response to PV IgG binding to KC have been obtained in the studies showing changes with phospholipase C, inositol 1,4,5-trisphosphate, transmembrane flux and intracellular levels of Ca2+, intracellular cAMP/cGMP ratios, and activity and intracellular location of protein kinase C (reviewed in Refs.	bind
42757	5	10018	7	11	NULL	NULL	NULL	statement 1	GP		activates					Ca2+	Chemical	transmembrane flux of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29466_s_350	10899159	A direct evidence of activation of second messenger systems in response to PV IgG binding to KC have been obtained in the studies showing changes with phospholipase C, inositol 1,4,5-trisphosphate, transmembrane flux and intracellular levels of Ca2+, intracellular cAMP/cGMP ratios, and activity and intracellular location of protein kinase C (reviewed in Refs.	bind
42758	6	10018	7	11	NULL	NULL	NULL	statement 1	GP		activates					Ca2+	Chemical	intracellular levels of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29466_s_350	10899159	A direct evidence of activation of second messenger systems in response to PV IgG binding to KC have been obtained in the studies showing changes with phospholipase C, inositol 1,4,5-trisphosphate, transmembrane flux and intracellular levels of Ca2+, intracellular cAMP/cGMP ratios, and activity and intracellular location of protein kinase C (reviewed in Refs.	bind
42759	7	10018	7	11	NULL	NULL	NULL	statement 1	GP		activates					cAMP/cGMP	Chemical	intracellular ratios of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29466_s_350	10899159	A direct evidence of activation of second messenger systems in response to PV IgG binding to KC have been obtained in the studies showing changes with phospholipase C, inositol 1,4,5-trisphosphate, transmembrane flux and intracellular levels of Ca2+, intracellular cAMP/cGMP ratios, and activity and intracellular location of protein kinase C (reviewed in Refs.	bind
42760	8	10018	7	11	NULL	NULL	NULL	statement 1	GP		activates					protein kinase C	GP	intracellular location of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29466_s_350	10899159	A direct evidence of activation of second messenger systems in response to PV IgG binding to KC have been obtained in the studies showing changes with phospholipase C, inositol 1,4,5-trisphosphate, transmembrane flux and intracellular levels of Ca2+, intracellular cAMP/cGMP ratios, and activity and intracellular location of protein kinase C (reviewed in Refs.	bind
42761	9	10018	7	11	NULL	NULL	NULL	statement 1	GP		activates					protein kinase C	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_38_29466_s_350	10899159	A direct evidence of activation of second messenger systems in response to PV IgG binding to KC have been obtained in the studies showing changes with phospholipase C, inositol 1,4,5-trisphosphate, transmembrane flux and intracellular levels of Ca2+, intracellular cAMP/cGMP ratios, and activity and intracellular location of protein kinase C (reviewed in Refs.	bind
35050	1	10019	6	11	NULL	NULL	NULL	apo E	GP		bind					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_963_s_232	7600129	A direct inhibition of apo E binding to the LDL receptor by apo CIII cannot be excluded.	bind
35051	2	10019	6	11	NULL	NULL	NULL	apo CIII	GP		inhibits		directly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_963_s_232	7600129	A direct inhibition of apo E binding to the LDL receptor by apo CIII cannot be excluded.	bind
42762	1	10019	7	11	NULL	NULL	NULL	apo E	GP		bind					LDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_963_s_232	7600129	A direct inhibition of apo E binding to the LDL receptor by apo CIII cannot be excluded.	bind
42763	2	10019	7	11	NULL	NULL	NULL	apo CIII	GP		inhibits		directly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_7_963_s_232	7600129	A direct inhibition of apo E binding to the LDL receptor by apo CIII cannot be excluded.	bind
35052	1	10020	6	11	NULL	NULL	NULL	CHIP	GP		interacts with		directly			AR	GP		NH2-terminal conserved motif		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_29_30643_s_248	15107424	A direct interaction between CHIP and the AR NH2-terminal conserved motif was confirmed in mammalian two-hybrid and GST affinity matrix binding assays, supporting the initial identification of CHIP in a yeast two-hybrid screen as a  bona fide AR-interacting protein.	bind
42764	1	10020	7	11	NULL	NULL	NULL	CHIP	GP		interacts with		directly			 AR	GP		NH2-terminal conserved motif		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_29_30643_s_248	15107424	A direct interaction between CHIP and the AR NH2-terminal conserved motif was confirmed in mammalian two-hybrid and GST affinity matrix binding assays, supporting the initial identification of CHIP in a yeast two-hybrid screen as a  bona fide AR-interacting protein.	bind
35053	1	10021	6	11	NULL	NULL	NULL	Swi5	GP		interacts 		directly			SWI/SNF	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4095_s_94	16705163	A direct interaction between Swi5 and SWI/SNF has been demonstrated in vitro ( ), and a  swi5 mutation eliminates SWI/SNF binding to  HO in vivo ( ).	bind
35054	2	10021	6	11	NULL	NULL	NULL	SWI/SNF	GP		bind					HO	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4095_s_94	16705163	A direct interaction between Swi5 and SWI/SNF has been demonstrated in vitro ( ), and a  swi5 mutation eliminates SWI/SNF binding to  HO in vivo ( ).	bind
35055	3	10021	6	11	NULL	NULL	NULL	Swi5	GP	mutant	eliminates					statement 2	Process				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4095_s_94	16705163	A direct interaction between Swi5 and SWI/SNF has been demonstrated in vitro ( ), and a  swi5 mutation eliminates SWI/SNF binding to  HO in vivo ( ).	bind
42765	1	10021	7	11	NULL	NULL	NULL	Swi5 	GP		interacts with		directly			SWI/SNF	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4095_s_94	16705163	A direct interaction between Swi5 and SWI/SNF has been demonstrated in vitro ( ), and a  swi5 mutation eliminates SWI/SNF binding to  HO in vivo ( ).	bind
42766	2	10021	7	11	NULL	NULL	NULL	SWI/SNF	GP		bind					HO	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4095_s_94	16705163	A direct interaction between Swi5 and SWI/SNF has been demonstrated in vitro ( ), and a  swi5 mutation eliminates SWI/SNF binding to  HO in vivo ( ).	bind
42767	3	10021	7	11	NULL	NULL	NULL	swi5	GP	mutant	eliminates					statement 2	Process				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_11_4095_s_94	16705163	A direct interaction between Swi5 and SWI/SNF has been demonstrated in vitro ( ), and a  swi5 mutation eliminates SWI/SNF binding to  HO in vivo ( ).	bind
35056	1	10022	6	11	NULL	NULL	NULL	gp32	GP		interacts with		directly	core domain		gp59	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_25236_s_47	11309384	A direct interaction between the core domain of gp32 and gp59 could destabilize the gp32-ssDNA interaction, which when followed by gp59 oligomer formation and binding to the helicase, results in displacement of gp32 from the DNA and loading of gp41 in its place.	bind
35057	2	10022	6	11	NULL	NULL	NULL	gp32	GP		interacts with					ssDNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_25236_s_47	11309384	A direct interaction between the core domain of gp32 and gp59 could destabilize the gp32-ssDNA interaction, which when followed by gp59 oligomer formation and binding to the helicase, results in displacement of gp32 from the DNA and loading of gp41 in its place.	bind
35058	3	10022	6	11	NULL	NULL	NULL	statement 1	Process		destabilize					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_25236_s_47	11309384	A direct interaction between the core domain of gp32 and gp59 could destabilize the gp32-ssDNA interaction, which when followed by gp59 oligomer formation and binding to the helicase, results in displacement of gp32 from the DNA and loading of gp41 in its place.	bind
35059	4	10022	6	11	NULL	NULL	NULL	gp59	GP		bind					helicase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_25236_s_47	11309384	A direct interaction between the core domain of gp32 and gp59 could destabilize the gp32-ssDNA interaction, which when followed by gp59 oligomer formation and binding to the helicase, results in displacement of gp32 from the DNA and loading of gp41 in its place.	bind
35060	5	10022	6	11	NULL	NULL	NULL	statement 3	Process		is followed by					gp59 oligomer	GP	formation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_25236_s_47	11309384	A direct interaction between the core domain of gp32 and gp59 could destabilize the gp32-ssDNA interaction, which when followed by gp59 oligomer formation and binding to the helicase, results in displacement of gp32 from the DNA and loading of gp41 in its place.	bind
35061	6	10022	6	11	NULL	NULL	NULL	statement 3	Process		is followed by					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_25236_s_47	11309384	A direct interaction between the core domain of gp32 and gp59 could destabilize the gp32-ssDNA interaction, which when followed by gp59 oligomer formation and binding to the helicase, results in displacement of gp32 from the DNA and loading of gp41 in its place.	bind
35062	7	10022	6	11	NULL	NULL	NULL	gp32	GP		is replaced by					gp41	GP				NULL	 in DNA	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_25236_s_47	11309384	A direct interaction between the core domain of gp32 and gp59 could destabilize the gp32-ssDNA interaction, which when followed by gp59 oligomer formation and binding to the helicase, results in displacement of gp32 from the DNA and loading of gp41 in its place.	bind
35063	8	10022	6	11	NULL	NULL	NULL	statement 4	Process		results in					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_25236_s_47	11309384	A direct interaction between the core domain of gp32 and gp59 could destabilize the gp32-ssDNA interaction, which when followed by gp59 oligomer formation and binding to the helicase, results in displacement of gp32 from the DNA and loading of gp41 in its place.	bind
42768	1	10022	7	11	NULL	NULL	NULL	gp32	GP		interacts with		directly	core domain		gp59	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_25236_s_47	11309384	A direct interaction between the core domain of gp32 and gp59 could destabilize the gp32-ssDNA interaction, which when followed by gp59 oligomer formation and binding to the helicase, results in displacement of gp32 from the DNA and loading of gp41 in its place.	bind
42769	2	10022	7	11	NULL	NULL	NULL	gp32	GP		interacts with					ssDNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_25236_s_47	11309384	A direct interaction between the core domain of gp32 and gp59 could destabilize the gp32-ssDNA interaction, which when followed by gp59 oligomer formation and binding to the helicase, results in displacement of gp32 from the DNA and loading of gp41 in its place.	bind
42770	3	10022	7	11	NULL	NULL	NULL	statement 1	Process		destabilize					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_25236_s_47	11309384	A direct interaction between the core domain of gp32 and gp59 could destabilize the gp32-ssDNA interaction, which when followed by gp59 oligomer formation and binding to the helicase, results in displacement of gp32 from the DNA and loading of gp41 in its place.	bind
42771	4	10022	7	11	NULL	NULL	NULL	gp59	GP		forms					oligomer	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_25236_s_47	11309384	A direct interaction between the core domain of gp32 and gp59 could destabilize the gp32-ssDNA interaction, which when followed by gp59 oligomer formation and binding to the helicase, results in displacement of gp32 from the DNA and loading of gp41 in its place.	bind
42772	5	10022	7	11	NULL	NULL	NULL	gp59	GP		bind					helicase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_25236_s_47	11309384	A direct interaction between the core domain of gp32 and gp59 could destabilize the gp32-ssDNA interaction, which when followed by gp59 oligomer formation and binding to the helicase, results in displacement of gp32 from the DNA and loading of gp41 in its place.	bind
42773	6	10022	7	11	NULL	NULL	NULL	statement 3	Process		is followed by					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_25236_s_47	11309384	A direct interaction between the core domain of gp32 and gp59 could destabilize the gp32-ssDNA interaction, which when followed by gp59 oligomer formation and binding to the helicase, results in displacement of gp32 from the DNA and loading of gp41 in its place.	bind
42774	7	10022	7	11	NULL	NULL	NULL	gp32	GP		is replaced by					gp41	GP				NULL	DNA	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_25236_s_47	11309384	A direct interaction between the core domain of gp32 and gp59 could destabilize the gp32-ssDNA interaction, which when followed by gp59 oligomer formation and binding to the helicase, results in displacement of gp32 from the DNA and loading of gp41 in its place.	bind
42775	8	10022	7	11	NULL	NULL	NULL	statement 5	Process		results in					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_25236_s_47	11309384	A direct interaction between the core domain of gp32 and gp59 could destabilize the gp32-ssDNA interaction, which when followed by gp59 oligomer formation and binding to the helicase, results in displacement of gp32 from the DNA and loading of gp41 in its place.	bind
35064	1	10023	6	11	NULL	NULL	NULL	Mot1	GP		interacts with		directly	DNA binding surface		TBP	GP		DNA binding surface		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_15_13216_s_478	12571241	A direct interaction between the DNA-binding surfaces of Mot1 and TBP can explain why the Mot1.TBP binary complex does not bind DNA.	bind
35065	2	10023	6	11	NULL	NULL	NULL	Mot1.TBP binary complex	GP		does not bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_15_13216_s_478	12571241	A direct interaction between the DNA-binding surfaces of Mot1 and TBP can explain why the Mot1.TBP binary complex does not bind DNA.	bind
42778	1	10023	7	11	NULL	NULL	NULL	Mot1	GP		interacts with		directly	DNA-binding surface		TBP	GP		DNA-binding surface		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_15_13216_s_478	12571241	A direct interaction between the DNA-binding surfaces of Mot1 and TBP can explain why the Mot1.TBP binary complex does not bind DNA.	bind
42779	2	10023	7	11	NULL	NULL	NULL	Mot1.TBP binary complex	GP		does not bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_15_13216_s_478	12571241	A direct interaction between the DNA-binding surfaces of Mot1 and TBP can explain why the Mot1.TBP binary complex does not bind DNA.	bind
35066	1	10024	6	11	NULL	NULL	NULL	Fir1p	GP	35S-labeled;;in vitro translated	bind			amino acids 173 - 876		GST-Sin1p	GP		N-terminus		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_26_9808_s_61	16788068	A direct interaction between the two proteins was confirmed by showing that 35S-labeled,  in vitro translated Fir1p (amino acids 173 - 876) bound GST-Sin1p fusion proteins derived from the N terminus of the protein, whereas GST alone did not bind ( Fig. 2).	bind
35067	2	10024	6	11	NULL	NULL	NULL	Fir1p	GP	35S-labeled;;in vitro translated	does not bind			amino acids 173 - 876		GST	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_26_9808_s_61	16788068	A direct interaction between the two proteins was confirmed by showing that 35S-labeled,  in vitro translated Fir1p (amino acids 173 - 876) bound GST-Sin1p fusion proteins derived from the N terminus of the protein, whereas GST alone did not bind ( Fig. 2).	bind
49331	3	10024	6	11	NULL	NULL	NULL	GST-Sin1p	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_26_9808_s_61	16788068	A direct interaction between the two proteins was confirmed by showing that 35S-labeled,  in vitro translated Fir1p (amino acids 173 - 876) bound GST-Sin1p fusion proteins derived from the N terminus of the protein, whereas GST alone did not bind ( Fig. 2).	bind
42781	1	10024	7	11	NULL	NULL	NULL	Fir1p	GP	35S-labeled;;in vitro translated	bind			amino acids 173 - 876		GST-Sin1p	GP	N-terminus			NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_26_9808_s_61	16788068	A direct interaction between the two proteins was confirmed by showing that 35S-labeled,  in vitro translated Fir1p (amino acids 173 - 876) bound GST-Sin1p fusion proteins derived from the N terminus of the protein, whereas GST alone did not bind ( Fig. 2).	bind
49332	2	10024	7	11	NULL	NULL	NULL	Fir1p	GP	35S-labeled;;in vitro translated	does not bind			amino acids 173 - 876		GST	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_26_9808_s_61	16788068	A direct interaction between the two proteins was confirmed by showing that 35S-labeled,  in vitro translated Fir1p (amino acids 173 - 876) bound GST-Sin1p fusion proteins derived from the N terminus of the protein, whereas GST alone did not bind ( Fig. 2).	bind
49334	3	10024	7	11	NULL	NULL	NULL	GST-Sin1p	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_26_9808_s_61	16788068	A direct interaction between the two proteins was confirmed by showing that 35S-labeled,  in vitro translated Fir1p (amino acids 173 - 876) bound GST-Sin1p fusion proteins derived from the N terminus of the protein, whereas GST alone did not bind ( Fig. 2).	bind
35068	1	10025	6	11	NULL	NULL	NULL	GTP	Chemical		bind					Cdc42p	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_20_5657_s_203	11598009	A direct interaction of Cla4p with the GTP-bound form of Cdc42p was shown by overlay and two-hybrid assays ( Cvrckova   et al., 1995;  Richman  et al., 1999).	bind
35069	2	10025	6	11	NULL	NULL	NULL	Cla4p	GP		interacts with		directly			statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_20_5657_s_203	11598009	A direct interaction of Cla4p with the GTP-bound form of Cdc42p was shown by overlay and two-hybrid assays ( Cvrckova   et al., 1995;  Richman  et al., 1999).	bind
42782	2	10025	7	11	NULL	NULL	NULL	Cla4p	GP		interacts with		directly			statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_20_5657_s_203	11598009	A direct interaction of Cla4p with the GTP-bound form of Cdc42p was shown by overlay and two-hybrid assays ( Cvrckova   et al., 1995;  Richman  et al., 1999).	bind
42783	1	10025	7	11	NULL	NULL	NULL	GTP	Chemical		bind					Cdc42p	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_20_5657_s_203	11598009	A direct interaction of Cla4p with the GTP-bound form of Cdc42p was shown by overlay and two-hybrid assays ( Cvrckova   et al., 1995;  Richman  et al., 1999).	bind
35498	1	10026	6	11	NULL	NULL	NULL	QacR	GP		bind					IR1 DNA	NucleicAcid			operator	NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
35519	2	10026	6	11	NULL	NULL	NULL	benzalkonium	Chemical		is a type of					QacA substrate	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
35520	3	10026	6	11	NULL	NULL	NULL	dequalinium	Chemical		is a type of					QacA substrate	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
35521	4	10026	6	11	NULL	NULL	NULL	ethidium bromide	Chemical		is a type of					QacA substrate	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
35522	5	10026	6	11	NULL	NULL	NULL	chlorhexidine	Chemical		is a type of					QacA substrate	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
35523	6	10026	6	11	NULL	NULL	NULL	rhodamine 6G	Chemical		is a type of					QacA substrate	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
35524	7	10026	6	11	NULL	NULL	NULL	QacR	GP		acts as a					sensor molecule	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
35525	8	10026	6	11	NULL	NULL	NULL	QacR	GP		facilitate					transcription	Process	increase in			NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
35526	9	10026	6	11	NULL	NULL	NULL	statement 8	Process		occurs in response to					toxic compounds	Chemical	presence of			NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
35527	10	10026	6	11	NULL	NULL	NULL	benzalkonium	Chemical		disrupts					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
35529	11	10026	6	11	NULL	NULL	NULL	dequalinium	Chemical		disrupts					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
35530	12	10026	6	11	NULL	NULL	NULL	ethidium bromide	Chemical		disrupts					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
35531	13	10026	6	11	NULL	NULL	NULL	chlorhexidine	Chemical		disrupts					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
35532	14	10026	6	11	NULL	NULL	NULL	rhodamine 6G	Chemical		disrupts					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
49335	15	10026	6	11	NULL	NULL	NULL	TetR	GP		acts as					sensor molecule 	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
49336	16	10026	6	11	NULL	NULL	NULL	ligand-bound QacR	GP		does not bind					DNA	NucleicAcid			operator	NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
57239	17	10026	6	11	NULL	NULL	NULL	TetR	GP		acts as					sensor molecule	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
42784	1	10026	7	11	NULL	NULL	NULL	QacR	GP		bind					IR1  DNA	NucleicAcid			operator	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
42785	2	10026	7	11	NULL	NULL	NULL	benzalkonium	Chemical		disrupts					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
42786	3	10026	7	11	NULL	NULL	NULL	dequalinium	Chemical		disrupts					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
42787	4	10026	7	11	NULL	NULL	NULL	ethidium bromide	Chemical		disrupts					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
42788	5	10026	7	11	NULL	NULL	NULL	chlorhexidine	Chemical		disrupts					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
42789	6	10026	7	11	NULL	NULL	NULL	rhodamine 6G	Chemical		disrupts					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
42790	7	10026	7	11	NULL	NULL	NULL	QacR	GP		acts as a					sensor molecule	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
42792	8	10026	7	11	NULL	NULL	NULL	TetR	GP		acts as a					sensor molecule	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
42794	10	10026	7	11	NULL	NULL	NULL	statement 7	Process		facilitate					transcription	Process	increase in			NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
42795	11	10026	7	11	NULL	NULL	NULL	statement 10	Process		occurs in response to					toxic compounds	Chemical	presence of			NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
42796	12	10026	7	11	NULL	NULL	NULL	ligand-bound QacR	GP		does not bind					DNA	NucleicAcid			operator	NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
42797	13	10026	7	11	NULL	NULL	NULL	benzalkonium	Chemical		is a type of					QacA substrate	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
42798	14	10026	7	11	NULL	NULL	NULL	dequalinium	Chemical		is a type of					QacA substrate	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
42799	15	10026	7	11	NULL	NULL	NULL	ethidium bromide	Chemical		is a type of					QacA substrate	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
42800	16	10026	7	11	NULL	NULL	NULL	chlorhexidine	Chemical		is a type of					QacA substrate	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
42801	17	10026	7	11	NULL	NULL	NULL	 rhodamine 6G	Chemical		is a type of					QacA substrate	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_66_4_671_s_514	12456787	A direct interaction of QacR with these inducing compounds was subsequently confirmed by the binding of QacR to IR1 operator DNA that had been disrupted in vitro by the separate addition of eight structurally diverse QacA substrates, including benzalkonium, dequalinium, ethidium bromide, chlorhexidine, and rhodamine 6G ( ) Thus, like TetR, QacR acts as a sensor molecule that can facilitate increases in transcription in response to the presence of toxic compounds because the ligand-bound form of this protein is incapable of binding operator DNA (Fig.  10A).	bind
35101	1	10028	6	11	NULL	NULL	NULL	YC-1	GP		bind					heme-depleted enzyme	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_53_1_123_s_8	9443939	A direct interaction of YC-1 with the heme group can be ruled out because YC-1 did not change the Soret absorption of basal or stimulated sGC and, in addition, still bound to the heme-depleted enzyme.	bind
35102	2	10028	6	11	NULL	NULL	NULL	YC-1	GP		does not interact with		directly			heme group	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_53_1_123_s_8	9443939	A direct interaction of YC-1 with the heme group can be ruled out because YC-1 did not change the Soret absorption of basal or stimulated sGC and, in addition, still bound to the heme-depleted enzyme.	bind
42802	1	10028	7	11	NULL	NULL	NULL	 YC-1 	GP		bind					heme-depleted enzyme	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_53_1_123_s_8	9443939	A direct interaction of YC-1 with the heme group can be ruled out because YC-1 did not change the Soret absorption of basal or stimulated sGC and, in addition, still bound to the heme-depleted enzyme.	bind
42803	2	10028	7	11	NULL	NULL	NULL	YC-1	GP		does not interact with		directly			heme group	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_53_1_123_s_8	9443939	A direct interaction of YC-1 with the heme group can be ruled out because YC-1 did not change the Soret absorption of basal or stimulated sGC and, in addition, still bound to the heme-depleted enzyme.	bind
35103	1	10029	6	11	NULL	NULL	NULL	E(Z)	GP	Drosophila	bind		directly			ESC	GP				NULL		NULL	NULL	NULL	NULL	gw60_genetics_159_3_1135_s_362	11729158	A direct link between E(Z) and histone deacetylation is suggested by the finding that the Drosophila E(Z) binds directly to ESC ( J ONES et al. 1998   ;	bind
49337	2	10029	6	11	NULL	NULL	NULL	E(Z)	GP		linked to		directly			histone	GP	deacetylation of			NULL		NULL	NULL	NULL	NULL	gw60_genetics_159_3_1135_s_362	11729158	A direct link between E(Z) and histone deacetylation is suggested by the finding that the Drosophila E(Z) binds directly to ESC ( J ONES et al. 1998   ;	bind
49338	3	10029	6	11	NULL	NULL	NULL	statement 1	Process		suggest					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_genetics_159_3_1135_s_362	11729158	A direct link between E(Z) and histone deacetylation is suggested by the finding that the Drosophila E(Z) binds directly to ESC ( J ONES et al. 1998   ;	bind
42804	1	10029	7	11	NULL	NULL	NULL	E(Z)	GP	Drosophila	binds		directly			ESC	GP				NULL		NULL	NULL	NULL	NULL	gw60_genetics_159_3_1135_s_362	11729158	A direct link between E(Z) and histone deacetylation is suggested by the finding that the Drosophila E(Z) binds directly to ESC ( J ONES et al. 1998   ;	bind
42805	2	10029	7	11	NULL	NULL	NULL	 E(Z) 	GP		linked to		directly			histone	GP	deacetylation of			NULL		NULL	NULL	NULL	NULL	gw60_genetics_159_3_1135_s_362	11729158	A direct link between E(Z) and histone deacetylation is suggested by the finding that the Drosophila E(Z) binds directly to ESC ( J ONES et al. 1998   ;	bind
42806	3	10029	7	11	NULL	NULL	NULL	statement 1	Process		suggests					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_genetics_159_3_1135_s_362	11729158	A direct link between E(Z) and histone deacetylation is suggested by the finding that the Drosophila E(Z) binds directly to ESC ( J ONES et al. 1998   ;	bind
35104	1	10030	6	11	NULL	NULL	NULL	protein 4.1	GP		bind					p55	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_10_5360_s_146	7890649	A direct measure of the protein 4.1  binding to p55 was obtained by determining the amount of  GPC-3-saturated protein 4.1 bound to p55-saturated alkali-stripped  membranes.	bind
42807	1	10030	7	11	NULL	NULL	NULL	protein 4.1	GP		bind					p55	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_10_5360_s_146	7890649	A direct measure of the protein 4.1  binding to p55 was obtained by determining the amount of  GPC-3-saturated protein 4.1 bound to p55-saturated alkali-stripped  membranes.	bind
35534	1	10031	6	11	NULL	NULL	NULL	IL-1ra analogs	GP		bind					IL-1R AcP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_38_22460_s_212	7673234	A direct measurement of binding of the IL-1ra analogs  to the IL-1R AcP is not possible because the accessory protein does not  bind IL-1 ligands except in the presence of the Type I  IL-1R( 37) .	bind
35535	2	10031	6	11	NULL	NULL	NULL	accessory protein	GP		bind					IL-1 ligands	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_38_22460_s_212	7673234	A direct measurement of binding of the IL-1ra analogs  to the IL-1R AcP is not possible because the accessory protein does not  bind IL-1 ligands except in the presence of the Type I  IL-1R( 37) .	bind
35536	3	10031	6	11	NULL	NULL	NULL	statement 2	Process		in presence of		only			Type I IL-1R	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_38_22460_s_212	7673234	A direct measurement of binding of the IL-1ra analogs  to the IL-1R AcP is not possible because the accessory protein does not  bind IL-1 ligands except in the presence of the Type I  IL-1R( 37) .	bind
42808	1	10031	7	11	NULL	NULL	NULL	IL-1ra analogs	GP		bind					IL-1R AcP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_38_22460_s_212	7673234	A direct measurement of binding of the IL-1ra analogs  to the IL-1R AcP is not possible because the accessory protein does not  bind IL-1 ligands except in the presence of the Type I  IL-1R( 37) .	bind
42809	2	10031	7	11	NULL	NULL	NULL	accessory protein	GP		bind					IL-1 ligands	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_38_22460_s_212	7673234	A direct measurement of binding of the IL-1ra analogs  to the IL-1R AcP is not possible because the accessory protein does not  bind IL-1 ligands except in the presence of the Type I  IL-1R( 37) .	bind
42810	3	10031	7	11	NULL	NULL	NULL	statement 2	Process		in the presence of 		only			Type I IL-1R	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_38_22460_s_212	7673234	A direct measurement of binding of the IL-1ra analogs  to the IL-1R AcP is not possible because the accessory protein does not  bind IL-1 ligands except in the presence of the Type I  IL-1R( 37) .	bind
35105	1	10032	6	11	NULL	NULL	NULL	myosin Ia	GP		bind					post-TGN vesicles	GP	ALPK1-carrying			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_27_25637_s_122	15883161	A direct overlap between ALPK1-labeled vesicular structures and myo1A-YFP staining is shown in  Fig. 4 H, strongly suggesting that myosin Ia binds to ALPK1-carrying post-TGN vesicles.	bind
42811	1	10032	7	11	NULL	NULL	NULL	myosin Ia	GP		binds to					post-TGN vesicles	GP	ALPK1-carrying			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_27_25637_s_122	15883161	A direct overlap between ALPK1-labeled vesicular structures and myo1A-YFP staining is shown in  Fig. 4 H, strongly suggesting that myosin Ia binds to ALPK1-carrying post-TGN vesicles.	bind
35106	1	10033	6	11	NULL	NULL	NULL	Cbl-N	GP	unphosphorylated	bind					ZAP-70	GP	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_39_24063_s_113	8798643	A direct phosphotyrosine-dependent binding between unphosphorylated Cbl-N and tyrosine-phosphorylated ZAP-70 strongly suggests the presence of a hitherto unidentified PTB domain within the transforming N-terminal region of Cbl, functionally analogous to PTB domains identified within the Shc adapter protein ( 31,  32,  33) and subsequently in insulin receptor substrate 1 ( 25).	bind
35107	2	10033	6	11	NULL	NULL	NULL	statement 1	Process		depends on		directly	PTB domain within N-terminal region		phosphotyrosine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_39_24063_s_113	8798643	A direct phosphotyrosine-dependent binding between unphosphorylated Cbl-N and tyrosine-phosphorylated ZAP-70 strongly suggests the presence of a hitherto unidentified PTB domain within the transforming N-terminal region of Cbl, functionally analogous to PTB domains identified within the Shc adapter protein ( 31,  32,  33) and subsequently in insulin receptor substrate 1 ( 25).	bind
35108	3	10033	6	11	NULL	NULL	NULL			unidentified	is present within			PTB domain		Cbl	GP		N-terminal region		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_39_24063_s_113	8798643	A direct phosphotyrosine-dependent binding between unphosphorylated Cbl-N and tyrosine-phosphorylated ZAP-70 strongly suggests the presence of a hitherto unidentified PTB domain within the transforming N-terminal region of Cbl, functionally analogous to PTB domains identified within the Shc adapter protein ( 31,  32,  33) and subsequently in insulin receptor substrate 1 ( 25).	bind
57242	4	10033	6	11	NULL	NULL	NULL	statement 1	Process		suggest		strongly			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_39_24063_s_113	8798643	A direct phosphotyrosine-dependent binding between unphosphorylated Cbl-N and tyrosine-phosphorylated ZAP-70 strongly suggests the presence of a hitherto unidentified PTB domain within the transforming N-terminal region of Cbl, functionally analogous to PTB domains identified within the Shc adapter protein ( 31,  32,  33) and subsequently in insulin receptor substrate 1 ( 25).	bind
57243	5	10033	6	11	NULL	NULL	NULL	statement 3	Process		is analogous to		functionally			Shc	GP		PTB domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_39_24063_s_113	8798643	A direct phosphotyrosine-dependent binding between unphosphorylated Cbl-N and tyrosine-phosphorylated ZAP-70 strongly suggests the presence of a hitherto unidentified PTB domain within the transforming N-terminal region of Cbl, functionally analogous to PTB domains identified within the Shc adapter protein ( 31,  32,  33) and subsequently in insulin receptor substrate 1 ( 25).	bind
57244	6	10033	6	11	NULL	NULL	NULL	statement 3	Process		is analogous to		functionally			insulin receptor substrate 1	GP		PTB domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_39_24063_s_113	8798643	A direct phosphotyrosine-dependent binding between unphosphorylated Cbl-N and tyrosine-phosphorylated ZAP-70 strongly suggests the presence of a hitherto unidentified PTB domain within the transforming N-terminal region of Cbl, functionally analogous to PTB domains identified within the Shc adapter protein ( 31,  32,  33) and subsequently in insulin receptor substrate 1 ( 25).	bind
57245	7	10033	6	11	NULL	NULL	NULL	Shc	GP		is a type of					adapter protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_39_24063_s_113	8798643	A direct phosphotyrosine-dependent binding between unphosphorylated Cbl-N and tyrosine-phosphorylated ZAP-70 strongly suggests the presence of a hitherto unidentified PTB domain within the transforming N-terminal region of Cbl, functionally analogous to PTB domains identified within the Shc adapter protein ( 31,  32,  33) and subsequently in insulin receptor substrate 1 ( 25).	bind
42812	1	10033	7	11	NULL	NULL	NULL	Cbl-N	GP	unphosphorylated 	bind					 ZAP-70	GP	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_39_24063_s_113	8798643	A direct phosphotyrosine-dependent binding between unphosphorylated Cbl-N and tyrosine-phosphorylated ZAP-70 strongly suggests the presence of a hitherto unidentified PTB domain within the transforming N-terminal region of Cbl, functionally analogous to PTB domains identified within the Shc adapter protein ( 31,  32,  33) and subsequently in insulin receptor substrate 1 ( 25).	bind
42813	2	10033	7	11	NULL	NULL	NULL	statement 1	Process		depends on		directly			phosphotyrosine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_39_24063_s_113	8798643	A direct phosphotyrosine-dependent binding between unphosphorylated Cbl-N and tyrosine-phosphorylated ZAP-70 strongly suggests the presence of a hitherto unidentified PTB domain within the transforming N-terminal region of Cbl, functionally analogous to PTB domains identified within the Shc adapter protein ( 31,  32,  33) and subsequently in insulin receptor substrate 1 ( 25).	bind
42814	3	10033	7	11	NULL	NULL	NULL	statement 1	Process		suggests		strongly			statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_39_24063_s_113	8798643	A direct phosphotyrosine-dependent binding between unphosphorylated Cbl-N and tyrosine-phosphorylated ZAP-70 strongly suggests the presence of a hitherto unidentified PTB domain within the transforming N-terminal region of Cbl, functionally analogous to PTB domains identified within the Shc adapter protein ( 31,  32,  33) and subsequently in insulin receptor substrate 1 ( 25).	bind
42815	4	10033	7	11	NULL	NULL	NULL	statement 7	Process		is analogous to		functionally			Shc	GP		PTB domains		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_39_24063_s_113	8798643	A direct phosphotyrosine-dependent binding between unphosphorylated Cbl-N and tyrosine-phosphorylated ZAP-70 strongly suggests the presence of a hitherto unidentified PTB domain within the transforming N-terminal region of Cbl, functionally analogous to PTB domains identified within the Shc adapter protein ( 31,  32,  33) and subsequently in insulin receptor substrate 1 ( 25).	bind
42816	5	10033	7	11	NULL	NULL	NULL	statement 7	Process		is analogous to		functionally			insulin receptor substrate 1	GP		PTB domains		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_39_24063_s_113	8798643	A direct phosphotyrosine-dependent binding between unphosphorylated Cbl-N and tyrosine-phosphorylated ZAP-70 strongly suggests the presence of a hitherto unidentified PTB domain within the transforming N-terminal region of Cbl, functionally analogous to PTB domains identified within the Shc adapter protein ( 31,  32,  33) and subsequently in insulin receptor substrate 1 ( 25).	bind
57240	6	10033	7	11	NULL	NULL	NULL	Shc	GP		is a type of					adapter protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_39_24063_s_113	8798643	A direct phosphotyrosine-dependent binding between unphosphorylated Cbl-N and tyrosine-phosphorylated ZAP-70 strongly suggests the presence of a hitherto unidentified PTB domain within the transforming N-terminal region of Cbl, functionally analogous to PTB domains identified within the Shc adapter protein ( 31,  32,  33) and subsequently in insulin receptor substrate 1 ( 25).	bind
57241	7	10033	7	11	NULL	NULL	NULL			unidentified	is present within			PTB domain		Cbl	GP		N-terminal region		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_39_24063_s_113	8798643	A direct phosphotyrosine-dependent binding between unphosphorylated Cbl-N and tyrosine-phosphorylated ZAP-70 strongly suggests the presence of a hitherto unidentified PTB domain within the transforming N-terminal region of Cbl, functionally analogous to PTB domains identified within the Shc adapter protein ( 31,  32,  33) and subsequently in insulin receptor substrate 1 ( 25).	bind
35109	1	10034	6	11	NULL	NULL	NULL	PDGFrbeta	GP		bind					integrin beta3 subunit	GP		extracellular domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_41_39882_s_292	12881526	A direct physical association between these two cell surface receptors likely plays a role in this cooperation, as the PDGFrbeta binds the extracellular domain of the integrin beta3 subunit in a manner that is independent of PDGFrbeta activation ( ).	bind
35110	2	10034	6	11	NULL	NULL	NULL	statement 1	Process		is independent of					PDGFrbeta	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_41_39882_s_292	12881526	A direct physical association between these two cell surface receptors likely plays a role in this cooperation, as the PDGFrbeta binds the extracellular domain of the integrin beta3 subunit in a manner that is independent of PDGFrbeta activation ( ).	bind
42817	1	10034	7	11	NULL	NULL	NULL	PDGFrbeta	GP		binds					integrin beta3 subunit 	GP		extracellular domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_41_39882_s_292	12881526	A direct physical association between these two cell surface receptors likely plays a role in this cooperation, as the PDGFrbeta binds the extracellular domain of the integrin beta3 subunit in a manner that is independent of PDGFrbeta activation ( ).	bind
42818	2	10034	7	11	NULL	NULL	NULL	statement 1	Process		is independent of					PDGFrbeta	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_41_39882_s_292	12881526	A direct physical association between these two cell surface receptors likely plays a role in this cooperation, as the PDGFrbeta binds the extracellular domain of the integrin beta3 subunit in a manner that is independent of PDGFrbeta activation ( ).	bind
35111	1	10035	6	11	NULL	NULL	NULL	OxyR	GP		bind					ahpC	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_7_2674_s_141	16547055	A direct regulation of  ahpC by OxyR was confirmed by DNA binding of OxyR to the  ahpC promoter region by using an electrophoretic mobility shift assay (Fig.  2C).	bind
35112	2	10035	6	11	NULL	NULL	NULL	OxyR	GP		regulates		directly			ahpC	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_7_2674_s_141	16547055	A direct regulation of  ahpC by OxyR was confirmed by DNA binding of OxyR to the  ahpC promoter region by using an electrophoretic mobility shift assay (Fig.  2C).	bind
42819	1	10035	7	11	NULL	NULL	NULL	OxyR 	GP		bind					ahpC	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_7_2674_s_141	16547055	A direct regulation of  ahpC by OxyR was confirmed by DNA binding of OxyR to the  ahpC promoter region by using an electrophoretic mobility shift assay (Fig.  2C).	bind
42820	2	10035	7	11	NULL	NULL	NULL	OxyR	GP		regulates		directly			ahpC	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_188_7_2674_s_141	16547055	A direct regulation of  ahpC by OxyR was confirmed by DNA binding of OxyR to the  ahpC promoter region by using an electrophoretic mobility shift assay (Fig.  2C).	bind
35537	1	10036	6	11	NULL	NULL	NULL	RFX	GP		belongs to			RFX5 subunit		methyl-DNA-binding proteins	GP	family of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_47_38914_s_214	16166088	A direct role for DNA methylation in the function of RFX may be possible because (i) the RFX5 subunit of RFX belongs to a family of methyl-DNA-binding proteins; (ii) C residue methylation is known not to inhibit the binding of RFX5 to a collagen gene promoter ( ); and (iii) RFX protects the methylation of the C residue immediately adjacent to its previously described  HLA-DRA promoter binding site ( Fig. 4,  E - G).	bind
35538	2	10036	6	11	NULL	NULL	NULL	RFX5	GP		bind					collagen gene	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_47_38914_s_214	16166088	A direct role for DNA methylation in the function of RFX may be possible because (i) the RFX5 subunit of RFX belongs to a family of methyl-DNA-binding proteins; (ii) C residue methylation is known not to inhibit the binding of RFX5 to a collagen gene promoter ( ); and (iii) RFX protects the methylation of the C residue immediately adjacent to its previously described  HLA-DRA promoter binding site ( Fig. 4,  E - G).	bind
35539	3	10036	6	11	NULL	NULL	NULL			methylation of	does not inhibit			C residue		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_47_38914_s_214	16166088	A direct role for DNA methylation in the function of RFX may be possible because (i) the RFX5 subunit of RFX belongs to a family of methyl-DNA-binding proteins; (ii) C residue methylation is known not to inhibit the binding of RFX5 to a collagen gene promoter ( ); and (iii) RFX protects the methylation of the C residue immediately adjacent to its previously described  HLA-DRA promoter binding site ( Fig. 4,  E - G).	bind
35543	4	10036	6	11	NULL	NULL	NULL	RFX	GP		protects							methylation of	C residue		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_47_38914_s_214	16166088	A direct role for DNA methylation in the function of RFX may be possible because (i) the RFX5 subunit of RFX belongs to a family of methyl-DNA-binding proteins; (ii) C residue methylation is known not to inhibit the binding of RFX5 to a collagen gene promoter ( ); and (iii) RFX protects the methylation of the C residue immediately adjacent to its previously described  HLA-DRA promoter binding site ( Fig. 4,  E - G).	bind
36454	5	10036	6	11	NULL	NULL	NULL	statement 4	Process		occurs					HLA-DR5	GP	adjacent to		promoter binding site	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_47_38914_s_214	16166088	A direct role for DNA methylation in the function of RFX may be possible because (i) the RFX5 subunit of RFX belongs to a family of methyl-DNA-binding proteins; (ii) C residue methylation is known not to inhibit the binding of RFX5 to a collagen gene promoter ( ); and (iii) RFX protects the methylation of the C residue immediately adjacent to its previously described  HLA-DRA promoter binding site ( Fig. 4,  E - G).	bind
42821	1	10036	7	11	NULL	NULL	NULL	RFX	GP		belongs to			 RFX5 subunit		methyl-DNA-binding proteins	GP	family of 			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_47_38914_s_214	16166088	A direct role for DNA methylation in the function of RFX may be possible because (i) the RFX5 subunit of RFX belongs to a family of methyl-DNA-binding proteins; (ii) C residue methylation is known not to inhibit the binding of RFX5 to a collagen gene promoter ( ); and (iii) RFX protects the methylation of the C residue immediately adjacent to its previously described  HLA-DRA promoter binding site ( Fig. 4,  E - G).	bind
42822	2	10036	7	11	NULL	NULL	NULL	RFX5	GP		bind					collagen gene	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_47_38914_s_214	16166088	A direct role for DNA methylation in the function of RFX may be possible because (i) the RFX5 subunit of RFX belongs to a family of methyl-DNA-binding proteins; (ii) C residue methylation is known not to inhibit the binding of RFX5 to a collagen gene promoter ( ); and (iii) RFX protects the methylation of the C residue immediately adjacent to its previously described  HLA-DRA promoter binding site ( Fig. 4,  E - G).	bind
42823	3	10036	7	11	NULL	NULL	NULL			methylation of	does not inhibit			C residue		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_47_38914_s_214	16166088	A direct role for DNA methylation in the function of RFX may be possible because (i) the RFX5 subunit of RFX belongs to a family of methyl-DNA-binding proteins; (ii) C residue methylation is known not to inhibit the binding of RFX5 to a collagen gene promoter ( ); and (iii) RFX protects the methylation of the C residue immediately adjacent to its previously described  HLA-DRA promoter binding site ( Fig. 4,  E - G).	bind
42824	4	10036	7	11	NULL	NULL	NULL	RFX	GP		protects							methylation of 	C residue		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_47_38914_s_214	16166088	A direct role for DNA methylation in the function of RFX may be possible because (i) the RFX5 subunit of RFX belongs to a family of methyl-DNA-binding proteins; (ii) C residue methylation is known not to inhibit the binding of RFX5 to a collagen gene promoter ( ); and (iii) RFX protects the methylation of the C residue immediately adjacent to its previously described  HLA-DRA promoter binding site ( Fig. 4,  E - G).	bind
42825	5	10036	7	11	NULL	NULL	NULL	statement 4	Process		occurs					HLA-DRA 	GP	adjacent to		promoter binding site	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_47_38914_s_214	16166088	A direct role for DNA methylation in the function of RFX may be possible because (i) the RFX5 subunit of RFX belongs to a family of methyl-DNA-binding proteins; (ii) C residue methylation is known not to inhibit the binding of RFX5 to a collagen gene promoter ( ); and (iii) RFX protects the methylation of the C residue immediately adjacent to its previously described  HLA-DRA promoter binding site ( Fig. 4,  E - G).	bind
35113	1	10037	6	11	NULL	NULL	NULL	AP1	GP		bind					AP3	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_devcell_2_2_135_s_93	11832239	A direct role of AP1 in regulating  AP3 is further supported by the finding that AP1 binds to the  AP3 promoter and that the binding site is required for normal activity of this promoter   (Hill et al., 1998  ; Tilly et al., 1998  ).	bind
35114	2	10037	6	11	NULL	NULL	NULL	AP3	GP		is required for				AP1 binding site of promoter	AP3 	GP	normal activity of 		promoter	NULL		NULL	NULL	NULL	NULL	gw60_devcell_2_2_135_s_93	11832239	A direct role of AP1 in regulating  AP3 is further supported by the finding that AP1 binds to the  AP3 promoter and that the binding site is required for normal activity of this promoter   (Hill et al., 1998  ; Tilly et al., 1998  ).	bind
42826	1	10037	7	11	NULL	NULL	NULL	 AP1	GP		binds to					AP3	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_devcell_2_2_135_s_93	11832239	A direct role of AP1 in regulating  AP3 is further supported by the finding that AP1 binds to the  AP3 promoter and that the binding site is required for normal activity of this promoter   (Hill et al., 1998  ; Tilly et al., 1998  ).	bind
42827	2	10037	7	11	NULL	NULL	NULL	AP3	GP		is required for				AP1 binding site of promoter	AP3	GP	normal activity of		 promoter	NULL		NULL	NULL	NULL	NULL	gw60_devcell_2_2_135_s_93	11832239	A direct role of AP1 in regulating  AP3 is further supported by the finding that AP1 binds to the  AP3 promoter and that the binding site is required for normal activity of this promoter   (Hill et al., 1998  ; Tilly et al., 1998  ).	bind
35115	1	10038	6	11	NULL	NULL	NULL	STAT1	GP		interacts with					p48	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_20070_s_171	9242679	A directed yeast two-hybrid transcription system detected interaction of STAT1 with p48 ( 31), and  in vitro mixing of crude lysates from cells overexpressing STAT1 and p48 showed apparent complex binding to DNA (38).	bind
49514	2	10038	6	11	NULL	NULL	NULL	statement 1	GP		bind					DNA	NucleicAcid				NULL	in vitro,crude lysates from cells overexpressing STAT1 and p48	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_20070_s_171	9242679	A directed yeast two-hybrid transcription system detected interaction of STAT1 with p48 ( 31), and  in vitro mixing of crude lysates from cells overexpressing STAT1 and p48 showed apparent complex binding to DNA (38).	bind
42828	1	10038	7	11	NULL	NULL	NULL	STAT1	GP		interacts with					p48	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_20070_s_171	9242679	A directed yeast two-hybrid transcription system detected interaction of STAT1 with p48 ( 31), and  in vitro mixing of crude lysates from cells overexpressing STAT1 and p48 showed apparent complex binding to DNA (38).	bind
42829	2	10038	7	11	NULL	NULL	NULL	statement 1	GP		bind					DNA	NucleicAcid				NULL	in vitro,crude lysates from cells overexpressing STAT1 and p48	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_20070_s_171	9242679	A directed yeast two-hybrid transcription system detected interaction of STAT1 with p48 ( 31), and  in vitro mixing of crude lysates from cells overexpressing STAT1 and p48 showed apparent complex binding to DNA (38).	bind
35116	1	10039	6	11	NULL	NULL	NULL	mPR	GP	recombinant	bind					progesterone	Chemical				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_annurevphysiol_67_0_335_s_302	15709962	A discrepancy was observed in the steroid- binding specificity in that recombinant  mPR in vitro bound progesterone only, whereas mPR expressed on the surface of breast  cancer cells responded to both progesterone and 20 S.	bind
35117	2	10039	6	11	NULL	NULL	NULL	mPR	GP		expressed on					breast cancer cells	Cell	surface of 			NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_67_0_335_s_302	15709962	A discrepancy was observed in the steroid- binding specificity in that recombinant  mPR in vitro bound progesterone only, whereas mPR expressed on the surface of breast  cancer cells responded to both progesterone and 20 S.	bind
35118	3	10039	6	11	NULL	NULL	NULL	statement 2	Cell		responds to					progesterone	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_67_0_335_s_302	15709962	A discrepancy was observed in the steroid- binding specificity in that recombinant  mPR in vitro bound progesterone only, whereas mPR expressed on the surface of breast  cancer cells responded to both progesterone and 20 S.	bind
35119	4	10039	6	11	NULL	NULL	NULL	statement 2	Cell		responds to					20 S	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_67_0_335_s_302	15709962	A discrepancy was observed in the steroid- binding specificity in that recombinant  mPR in vitro bound progesterone only, whereas mPR expressed on the surface of breast  cancer cells responded to both progesterone and 20 S.	bind
42830	1	10039	7	11	NULL	NULL	NULL	mPR	GP	recombinant	bind					progesterone	Chemical				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_annurevphysiol_67_0_335_s_302	15709962	A discrepancy was observed in the steroid- binding specificity in that recombinant  mPR in vitro bound progesterone only, whereas mPR expressed on the surface of breast  cancer cells responded to both progesterone and 20 S.	bind
42831	2	10039	7	11	NULL	NULL	NULL	mPR	GP		expressed on					breast cancer cells 	Cell	surface of			NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_67_0_335_s_302	15709962	A discrepancy was observed in the steroid- binding specificity in that recombinant  mPR in vitro bound progesterone only, whereas mPR expressed on the surface of breast  cancer cells responded to both progesterone and 20 S.	bind
42832	3	10039	7	11	NULL	NULL	NULL	statement 2	Cell		respond to					progesterone	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_67_0_335_s_302	15709962	A discrepancy was observed in the steroid- binding specificity in that recombinant  mPR in vitro bound progesterone only, whereas mPR expressed on the surface of breast  cancer cells responded to both progesterone and 20 S.	bind
42833	4	10039	7	11	NULL	NULL	NULL	statement 2	Cell		respond to					20 S	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_67_0_335_s_302	15709962	A discrepancy was observed in the steroid- binding specificity in that recombinant  mPR in vitro bound progesterone only, whereas mPR expressed on the surface of breast  cancer cells responded to both progesterone and 20 S.	bind
35590	1	10040	6	11	NULL	NULL	NULL	P2	CellComponent		bind					Pex1p	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_5_761_s_129	15738267	A discrete group of detergent-insoluble membrane proteins, including the P1-associated forms of Pex1p, PI(4)P-bp, PI(4,5)P2-bp, and GTP-bp ( Fig. 4 A) and the P2-bound forms of Pex1p, Pex6p, PI(4)P-bp, and PI(4,5)P2-bp ( Fig. 4 B), floated to the low-density fractions 5 - 9 and peaked in fraction 7 of the gradient.	bind
35591	2	10040	6	11	NULL	NULL	NULL	P2	CellComponent		bind					Pex6p	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_5_761_s_129	15738267	A discrete group of detergent-insoluble membrane proteins, including the P1-associated forms of Pex1p, PI(4)P-bp, PI(4,5)P2-bp, and GTP-bp ( Fig. 4 A) and the P2-bound forms of Pex1p, Pex6p, PI(4)P-bp, and PI(4,5)P2-bp ( Fig. 4 B), floated to the low-density fractions 5 - 9 and peaked in fraction 7 of the gradient.	bind
35592	3	10040	6	11	NULL	NULL	NULL	P2	CellComponent		bind					PI(4)P-bp	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_5_761_s_129	15738267	A discrete group of detergent-insoluble membrane proteins, including the P1-associated forms of Pex1p, PI(4)P-bp, PI(4,5)P2-bp, and GTP-bp ( Fig. 4 A) and the P2-bound forms of Pex1p, Pex6p, PI(4)P-bp, and PI(4,5)P2-bp ( Fig. 4 B), floated to the low-density fractions 5 - 9 and peaked in fraction 7 of the gradient.	bind
35593	4	10040	6	11	NULL	NULL	NULL	P2	CellComponent		bind					PI(4,5)P2-bp	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_5_761_s_129	15738267	A discrete group of detergent-insoluble membrane proteins, including the P1-associated forms of Pex1p, PI(4)P-bp, PI(4,5)P2-bp, and GTP-bp ( Fig. 4 A) and the P2-bound forms of Pex1p, Pex6p, PI(4)P-bp, and PI(4,5)P2-bp ( Fig. 4 B), floated to the low-density fractions 5 - 9 and peaked in fraction 7 of the gradient.	bind
35594	5	10040	6	11	NULL	NULL	NULL	Pex1p	GP		is a type of					membrane protein	GP	detergent insoluble			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_5_761_s_129	15738267	A discrete group of detergent-insoluble membrane proteins, including the P1-associated forms of Pex1p, PI(4)P-bp, PI(4,5)P2-bp, and GTP-bp ( Fig. 4 A) and the P2-bound forms of Pex1p, Pex6p, PI(4)P-bp, and PI(4,5)P2-bp ( Fig. 4 B), floated to the low-density fractions 5 - 9 and peaked in fraction 7 of the gradient.	bind
35595	6	10040	6	11	NULL	NULL	NULL	Pex6p	GP		is a type of					membrane protein	GP	detergent insoluble			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_5_761_s_129	15738267	A discrete group of detergent-insoluble membrane proteins, including the P1-associated forms of Pex1p, PI(4)P-bp, PI(4,5)P2-bp, and GTP-bp ( Fig. 4 A) and the P2-bound forms of Pex1p, Pex6p, PI(4)P-bp, and PI(4,5)P2-bp ( Fig. 4 B), floated to the low-density fractions 5 - 9 and peaked in fraction 7 of the gradient.	bind
35596	7	10040	6	11	NULL	NULL	NULL	PI(4)P-bp	GP		is a type of					membrane protein	GP	detergent insoluble			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_5_761_s_129	15738267	A discrete group of detergent-insoluble membrane proteins, including the P1-associated forms of Pex1p, PI(4)P-bp, PI(4,5)P2-bp, and GTP-bp ( Fig. 4 A) and the P2-bound forms of Pex1p, Pex6p, PI(4)P-bp, and PI(4,5)P2-bp ( Fig. 4 B), floated to the low-density fractions 5 - 9 and peaked in fraction 7 of the gradient.	bind
35597	8	10040	6	11	NULL	NULL	NULL	PI(4,5)P2-bp	GP		is a type of					membrane protein	GP	detergent insoluble			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_5_761_s_129	15738267	A discrete group of detergent-insoluble membrane proteins, including the P1-associated forms of Pex1p, PI(4)P-bp, PI(4,5)P2-bp, and GTP-bp ( Fig. 4 A) and the P2-bound forms of Pex1p, Pex6p, PI(4)P-bp, and PI(4,5)P2-bp ( Fig. 4 B), floated to the low-density fractions 5 - 9 and peaked in fraction 7 of the gradient.	bind
35598	9	10040	6	11	NULL	NULL	NULL	P1	CellComponent		associates with					Pex1p	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_5_761_s_129	15738267	A discrete group of detergent-insoluble membrane proteins, including the P1-associated forms of Pex1p, PI(4)P-bp, PI(4,5)P2-bp, and GTP-bp ( Fig. 4 A) and the P2-bound forms of Pex1p, Pex6p, PI(4)P-bp, and PI(4,5)P2-bp ( Fig. 4 B), floated to the low-density fractions 5 - 9 and peaked in fraction 7 of the gradient.	bind
35599	10	10040	6	11	NULL	NULL	NULL	P1	CellComponent		associates with					PI(4)P-bp	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_5_761_s_129	15738267	A discrete group of detergent-insoluble membrane proteins, including the P1-associated forms of Pex1p, PI(4)P-bp, PI(4,5)P2-bp, and GTP-bp ( Fig. 4 A) and the P2-bound forms of Pex1p, Pex6p, PI(4)P-bp, and PI(4,5)P2-bp ( Fig. 4 B), floated to the low-density fractions 5 - 9 and peaked in fraction 7 of the gradient.	bind
35600	11	10040	6	11	NULL	NULL	NULL	P1	CellComponent		associates with					PI(4,5)P2-bp	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_5_761_s_129	15738267	A discrete group of detergent-insoluble membrane proteins, including the P1-associated forms of Pex1p, PI(4)P-bp, PI(4,5)P2-bp, and GTP-bp ( Fig. 4 A) and the P2-bound forms of Pex1p, Pex6p, PI(4)P-bp, and PI(4,5)P2-bp ( Fig. 4 B), floated to the low-density fractions 5 - 9 and peaked in fraction 7 of the gradient.	bind
35601	12	10040	6	11	NULL	NULL	NULL	P1	CellComponent		associates with					GTP-bp	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_5_761_s_129	15738267	A discrete group of detergent-insoluble membrane proteins, including the P1-associated forms of Pex1p, PI(4)P-bp, PI(4,5)P2-bp, and GTP-bp ( Fig. 4 A) and the P2-bound forms of Pex1p, Pex6p, PI(4)P-bp, and PI(4,5)P2-bp ( Fig. 4 B), floated to the low-density fractions 5 - 9 and peaked in fraction 7 of the gradient.	bind
42834	1	10040	7	11	NULL	NULL	NULL	P1	CellComponent		associate with					Pex1p	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_5_761_s_129	15738267	A discrete group of detergent-insoluble membrane proteins, including the P1-associated forms of Pex1p, PI(4)P-bp, PI(4,5)P2-bp, and GTP-bp ( Fig. 4 A) and the P2-bound forms of Pex1p, Pex6p, PI(4)P-bp, and PI(4,5)P2-bp ( Fig. 4 B), floated to the low-density fractions 5 - 9 and peaked in fraction 7 of the gradient.	bind
42835	2	10040	7	11	NULL	NULL	NULL	Pex1p	GP		is a type of					 membrane protein	GP	 detergent-insoluble			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_5_761_s_129	15738267	A discrete group of detergent-insoluble membrane proteins, including the P1-associated forms of Pex1p, PI(4)P-bp, PI(4,5)P2-bp, and GTP-bp ( Fig. 4 A) and the P2-bound forms of Pex1p, Pex6p, PI(4)P-bp, and PI(4,5)P2-bp ( Fig. 4 B), floated to the low-density fractions 5 - 9 and peaked in fraction 7 of the gradient.	bind
42836	3	10040	7	11	NULL	NULL	NULL	PI(4)P-bp	GP		is a type of					 membrane protein	GP	detergent-insoluble			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_5_761_s_129	15738267	A discrete group of detergent-insoluble membrane proteins, including the P1-associated forms of Pex1p, PI(4)P-bp, PI(4,5)P2-bp, and GTP-bp ( Fig. 4 A) and the P2-bound forms of Pex1p, Pex6p, PI(4)P-bp, and PI(4,5)P2-bp ( Fig. 4 B), floated to the low-density fractions 5 - 9 and peaked in fraction 7 of the gradient.	bind
42837	4	10040	7	11	NULL	NULL	NULL	PI(4,5)P2-bp	GP		is a type of					 membrane protein	GP	detergent-insoluble			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_5_761_s_129	15738267	A discrete group of detergent-insoluble membrane proteins, including the P1-associated forms of Pex1p, PI(4)P-bp, PI(4,5)P2-bp, and GTP-bp ( Fig. 4 A) and the P2-bound forms of Pex1p, Pex6p, PI(4)P-bp, and PI(4,5)P2-bp ( Fig. 4 B), floated to the low-density fractions 5 - 9 and peaked in fraction 7 of the gradient.	bind
42838	5	10040	7	11	NULL	NULL	NULL	GTP-bp	GP		is a type of					 membrane protein	GP	detergent-insoluble			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_5_761_s_129	15738267	A discrete group of detergent-insoluble membrane proteins, including the P1-associated forms of Pex1p, PI(4)P-bp, PI(4,5)P2-bp, and GTP-bp ( Fig. 4 A) and the P2-bound forms of Pex1p, Pex6p, PI(4)P-bp, and PI(4,5)P2-bp ( Fig. 4 B), floated to the low-density fractions 5 - 9 and peaked in fraction 7 of the gradient.	bind
42839	6	10040	7	11	NULL	NULL	NULL	P2	CellComponent		bind					Pex1p	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_5_761_s_129	15738267	A discrete group of detergent-insoluble membrane proteins, including the P1-associated forms of Pex1p, PI(4)P-bp, PI(4,5)P2-bp, and GTP-bp ( Fig. 4 A) and the P2-bound forms of Pex1p, Pex6p, PI(4)P-bp, and PI(4,5)P2-bp ( Fig. 4 B), floated to the low-density fractions 5 - 9 and peaked in fraction 7 of the gradient.	bind
49861	7	10040	7	11	NULL	NULL	NULL	P1	CellComponent		associate with					PI(4)P-bp	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_5_761_s_129	15738267	A discrete group of detergent-insoluble membrane proteins, including the P1-associated forms of Pex1p, PI(4)P-bp, PI(4,5)P2-bp, and GTP-bp ( Fig. 4 A) and the P2-bound forms of Pex1p, Pex6p, PI(4)P-bp, and PI(4,5)P2-bp ( Fig. 4 B), floated to the low-density fractions 5 - 9 and peaked in fraction 7 of the gradient.	bind
49862	8	10040	7	11	NULL	NULL	NULL	P1	CellComponent		associate with					PI(4,5)P2-bp	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_5_761_s_129	15738267	A discrete group of detergent-insoluble membrane proteins, including the P1-associated forms of Pex1p, PI(4)P-bp, PI(4,5)P2-bp, and GTP-bp ( Fig. 4 A) and the P2-bound forms of Pex1p, Pex6p, PI(4)P-bp, and PI(4,5)P2-bp ( Fig. 4 B), floated to the low-density fractions 5 - 9 and peaked in fraction 7 of the gradient.	bind
49863	9	10040	7	11	NULL	NULL	NULL	P1	CellComponent		associate with					GTP-bp	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_5_761_s_129	15738267	A discrete group of detergent-insoluble membrane proteins, including the P1-associated forms of Pex1p, PI(4)P-bp, PI(4,5)P2-bp, and GTP-bp ( Fig. 4 A) and the P2-bound forms of Pex1p, Pex6p, PI(4)P-bp, and PI(4,5)P2-bp ( Fig. 4 B), floated to the low-density fractions 5 - 9 and peaked in fraction 7 of the gradient.	bind
49864	10	10040	7	11	NULL	NULL	NULL	P2	CellComponent		bind					Pex6p	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_5_761_s_129	15738267	A discrete group of detergent-insoluble membrane proteins, including the P1-associated forms of Pex1p, PI(4)P-bp, PI(4,5)P2-bp, and GTP-bp ( Fig. 4 A) and the P2-bound forms of Pex1p, Pex6p, PI(4)P-bp, and PI(4,5)P2-bp ( Fig. 4 B), floated to the low-density fractions 5 - 9 and peaked in fraction 7 of the gradient.	bind
49865	11	10040	7	11	NULL	NULL	NULL	P2	CellComponent		bind					PI(4)P-bp	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_5_761_s_129	15738267	A discrete group of detergent-insoluble membrane proteins, including the P1-associated forms of Pex1p, PI(4)P-bp, PI(4,5)P2-bp, and GTP-bp ( Fig. 4 A) and the P2-bound forms of Pex1p, Pex6p, PI(4)P-bp, and PI(4,5)P2-bp ( Fig. 4 B), floated to the low-density fractions 5 - 9 and peaked in fraction 7 of the gradient.	bind
49866	12	10040	7	11	NULL	NULL	NULL	P2	CellComponent		bind					PI(4,5)P2-bp	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_5_761_s_129	15738267	A discrete group of detergent-insoluble membrane proteins, including the P1-associated forms of Pex1p, PI(4)P-bp, PI(4,5)P2-bp, and GTP-bp ( Fig. 4 A) and the P2-bound forms of Pex1p, Pex6p, PI(4)P-bp, and PI(4,5)P2-bp ( Fig. 4 B), floated to the low-density fractions 5 - 9 and peaked in fraction 7 of the gradient.	bind
35120	1	10041	6	11	NULL	NULL	NULL	BACE	GP		bind					GGA protein	GP		VHS domain		NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-cell-sci_117_pt-22_15466887_s_4	15466887	A DISLL sequence near the BACE  C-terminus mediates binding of BACE to the VHS domains of Golgi-localized  gamma-ear-containing ARF-binding (GGA) proteins, which are involved in  the sorting of proteins to endosomes.	bind
35121	2	10041	6	11	NULL	NULL	NULL	GGA	GP		is 					Golgi-localized gamma-ear-containing ARF-binding proteins	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-cell-sci_117_pt-22_15466887_s_4	15466887	A DISLL sequence near the BACE  C-terminus mediates binding of BACE to the VHS domains of Golgi-localized  gamma-ear-containing ARF-binding (GGA) proteins, which are involved in  the sorting of proteins to endosomes.	bind
35122	3	10041	6	11	NULL	NULL	NULL	BACE	GP		mediates			DISLL sequence near C terminus		statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-cell-sci_117_pt-22_15466887_s_4	15466887	A DISLL sequence near the BACE  C-terminus mediates binding of BACE to the VHS domains of Golgi-localized  gamma-ear-containing ARF-binding (GGA) proteins, which are involved in  the sorting of proteins to endosomes.	bind
49515	4	10041	6	11	NULL	NULL	NULL	proteins	GP		sorted to					endosomes	CellComponent				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-cell-sci_117_pt-22_15466887_s_4	15466887	A DISLL sequence near the BACE  C-terminus mediates binding of BACE to the VHS domains of Golgi-localized  gamma-ear-containing ARF-binding (GGA) proteins, which are involved in  the sorting of proteins to endosomes.	bind
49516	5	10041	6	11	NULL	NULL	NULL	GGA	GP		is involved in					statement 4	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-cell-sci_117_pt-22_15466887_s_4	15466887	A DISLL sequence near the BACE  C-terminus mediates binding of BACE to the VHS domains of Golgi-localized  gamma-ear-containing ARF-binding (GGA) proteins, which are involved in  the sorting of proteins to endosomes.	bind
42861	1	10041	7	11	NULL	NULL	NULL	BACE	GP		bind					GGA proteins	GP		VHS domain		NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-cell-sci_117_pt-22_15466887_s_4	15466887	A DISLL sequence near the BACE  C-terminus mediates binding of BACE to the VHS domains of Golgi-localized  gamma-ear-containing ARF-binding (GGA) proteins, which are involved in  the sorting of proteins to endosomes.	bind
42862	2	10041	7	11	NULL	NULL	NULL	BACE	GP		mediates			DISLL sequence near C-terminus		statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-cell-sci_117_pt-22_15466887_s_4	15466887	A DISLL sequence near the BACE  C-terminus mediates binding of BACE to the VHS domains of Golgi-localized  gamma-ear-containing ARF-binding (GGA) proteins, which are involved in  the sorting of proteins to endosomes.	bind
42863	4	10041	7	11	NULL	NULL	NULL	GGA	GP		is involved in					statement 3	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-cell-sci_117_pt-22_15466887_s_4	15466887	A DISLL sequence near the BACE  C-terminus mediates binding of BACE to the VHS domains of Golgi-localized  gamma-ear-containing ARF-binding (GGA) proteins, which are involved in  the sorting of proteins to endosomes.	bind
42864	3	10041	7	11	NULL	NULL	NULL	proteins	GP		sorted to					endosomes	CellComponent				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-cell-sci_117_pt-22_15466887_s_4	15466887	A DISLL sequence near the BACE  C-terminus mediates binding of BACE to the VHS domains of Golgi-localized  gamma-ear-containing ARF-binding (GGA) proteins, which are involved in  the sorting of proteins to endosomes.	bind
42865	5	10041	7	11	NULL	NULL	NULL	GGA	GP		is					Golgi-localized gamma-ear-containing ARF-binding proteins	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-cell-sci_117_pt-22_15466887_s_4	15466887	A DISLL sequence near the BACE  C-terminus mediates binding of BACE to the VHS domains of Golgi-localized  gamma-ear-containing ARF-binding (GGA) proteins, which are involved in  the sorting of proteins to endosomes.	bind
35138	1	10042	6	11	NULL	NULL	NULL	Lp(a)	GP		bind					TRL particles	GP	larger			NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_42_12_2058_s_11	11734579	A disproportionate amount of Lp[a was bound to the larger TRL particles.	bind
42866	1	10042	7	11	NULL	NULL	NULL	Lp[a	GP		bind					TRL particles	GP	larger			NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_42_12_2058_s_11	11734579	A disproportionate amount of Lp[a was bound to the larger TRL particles.	bind
35139	1	10043	6	11	NULL	NULL	NULL	LRP-2	GP	radiolabeled	bind					SVS-II	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_9_5557_s_136	10026171	A dissociation constant ( K d) of 10.4  plus-or-minus  4.9 nM ( n = 6) was determined for the binding of radiolabeled LRP-2 to SVS-II from the best fit of the data to a single class of binding sites model.	bind
42867	1	10043	7	11	NULL	NULL	NULL	 LRP-2	GP	radiolabeled 	bind					SVS-II	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_9_5557_s_136	10026171	A dissociation constant ( K d) of 10.4  plus-or-minus  4.9 nM ( n = 6) was determined for the binding of radiolabeled LRP-2 to SVS-II from the best fit of the data to a single class of binding sites model.	bind
35140	1	10044	6	11	NULL	NULL	NULL	LTP-like basic protein	GP	Oat	bind					oleic acid	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_structure_3_2_189_s_149	7735835	A dissociation constant of 3.5x10-6 M has been reported for the binding of oleic acid by an LTP-like basic protein from oat  [13]  .	bind
42868	1	10044	7	11	NULL	NULL	NULL	LTP-like basic protein 	GP	Oat	bind					oleic acid	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_structure_3_2_189_s_149	7735835	A dissociation constant of 3.5x10-6 M has been reported for the binding of oleic acid by an LTP-like basic protein from oat  [13]  .	bind
35141	1	10045	6	11	NULL	NULL	NULL	CD36	GP		bind					HDL	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_40_30794_s_245	10896940	A dissociation of efflux from binding is also indicated by the finding that CD36 can bind HDL but it does not facilitate cholesterol efflux ( 7).	bind
35142	2	10045	6	11	NULL	NULL	NULL	CD36	GP		does not facilitate					cholesterol efflux	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_40_30794_s_245	10896940	A dissociation of efflux from binding is also indicated by the finding that CD36 can bind HDL but it does not facilitate cholesterol efflux ( 7).	bind
42869	1	10045	7	11	NULL	NULL	NULL	CD36	GP		bind					HDL	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_40_30794_s_245	10896940	A dissociation of efflux from binding is also indicated by the finding that CD36 can bind HDL but it does not facilitate cholesterol efflux ( 7).	bind
42870	2	10045	7	11	NULL	NULL	NULL	CD36	GP		does not facilitate					cholesterol efflux	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_40_30794_s_245	10896940	A dissociation of efflux from binding is also indicated by the finding that CD36 can bind HDL but it does not facilitate cholesterol efflux ( 7).	bind
35143	1	10046	6	11	NULL	NULL	NULL	glucose oxidase	GP		oxidizes					hydrogen peroxide	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_anal-chem_75_5_12641231_s_8	12641231	A distinct current increase following the oxidation  of hydrogen peroxide produced by the enzymatic reaction of glucose oxidase  was observed, which indicates that the capture proteins could actually  bind the target proteins.	bind
42871	1	10046	7	11	NULL	NULL	NULL	glucose oxidase	GP		oxidizes					hydrogen peroxide	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_anal-chem_75_5_12641231_s_8	12641231	A distinct current increase following the oxidation  of hydrogen peroxide produced by the enzymatic reaction of glucose oxidase  was observed, which indicates that the capture proteins could actually  bind the target proteins.	bind
35144	1	10047	6	11	NULL	NULL	NULL	anti-galactan monoclonal antibody	GP		bind					beta-(1 6)-galactosyl ligand	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_14_8209_s_85	8626513	A distinct difference can be seen on the one hand between the  anti-galactan monoclonal antibodies binding to  beta-(1 6)-galactosyl ligands and on the other hand the  anti-dextran monoclonal antibodies binding to alpha-(1 6)-glucosyl  ligands (  Table 6 and   Table 7 and   Fig. 5 and  Fig. 6 ).	bind
35145	2	10047	6	11	NULL	NULL	NULL	anti-dextran monoclonal antibody	GP		bind					alpha-(1 6)-glucosyl ligand	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_14_8209_s_85	8626513	A distinct difference can be seen on the one hand between the  anti-galactan monoclonal antibodies binding to  beta-(1 6)-galactosyl ligands and on the other hand the  anti-dextran monoclonal antibodies binding to alpha-(1 6)-glucosyl  ligands (  Table 6 and   Table 7 and   Fig. 5 and  Fig. 6 ).	bind
42872	1	10047	7	11	NULL	NULL	NULL	anti-galactan monoclonal antibodies	GP		bind					beta-(1 6)-galactosyl ligands 	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_14_8209_s_85	8626513	A distinct difference can be seen on the one hand between the  anti-galactan monoclonal antibodies binding to  beta-(1 6)-galactosyl ligands and on the other hand the  anti-dextran monoclonal antibodies binding to alpha-(1 6)-glucosyl  ligands (  Table 6 and   Table 7 and   Fig. 5 and  Fig. 6 ).	bind
42873	2	10047	7	11	NULL	NULL	NULL	anti-dextran monoclonal antibodies	GP		bind					alpha-(1 6)-glucosyl ligands	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_14_8209_s_85	8626513	A distinct difference can be seen on the one hand between the  anti-galactan monoclonal antibodies binding to  beta-(1 6)-galactosyl ligands and on the other hand the  anti-dextran monoclonal antibodies binding to alpha-(1 6)-glucosyl  ligands (  Table 6 and   Table 7 and   Fig. 5 and  Fig. 6 ).	bind
35152	1	10048	6	11	NULL	NULL	NULL	Exo III	GP		bind					MutY	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_25_22605_s_407	11960995	A distinct feature of Exo III, is that, unlike Endo IV and MutM, it does not bind to the DNA duplex under the conditions used; however, Exo III does bind to the MutY.	bind
35153	2	10048	6	11	NULL	NULL	NULL	Endo IV	GP		bind					DNA duplex	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_25_22605_s_407	11960995	A distinct feature of Exo III, is that, unlike Endo IV and MutM, it does not bind to the DNA duplex under the conditions used; however, Exo III does bind to the MutY.	bind
35154	3	10048	6	11	NULL	NULL	NULL	MutM	GP		bind					DNA duplex	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_25_22605_s_407	11960995	A distinct feature of Exo III, is that, unlike Endo IV and MutM, it does not bind to the DNA duplex under the conditions used; however, Exo III does bind to the MutY.	bind
35155	4	10048	6	11	NULL	NULL	NULL	Exo III	GP		does not bind					DNA duplex	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_25_22605_s_407	11960995	A distinct feature of Exo III, is that, unlike Endo IV and MutM, it does not bind to the DNA duplex under the conditions used; however, Exo III does bind to the MutY.	bind
42874	1	10048	7	11	NULL	NULL	NULL	 Exo III	GP		does not bind					DNA duplex	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_25_22605_s_407	11960995	A distinct feature of Exo III, is that, unlike Endo IV and MutM, it does not bind to the DNA duplex under the conditions used; however, Exo III does bind to the MutY.	bind
42875	2	10048	7	11	NULL	NULL	NULL	Endo IV	GP		bind					DNA duplex	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_25_22605_s_407	11960995	A distinct feature of Exo III, is that, unlike Endo IV and MutM, it does not bind to the DNA duplex under the conditions used; however, Exo III does bind to the MutY.	bind
42876	3	10048	7	11	NULL	NULL	NULL	MutM	GP		bind					DNA duplex	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_25_22605_s_407	11960995	A distinct feature of Exo III, is that, unlike Endo IV and MutM, it does not bind to the DNA duplex under the conditions used; however, Exo III does bind to the MutY.	bind
42877	4	10048	7	11	NULL	NULL	NULL	Exo III	GP		bind					MutY	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_25_22605_s_407	11960995	A distinct feature of Exo III, is that, unlike Endo IV and MutM, it does not bind to the DNA duplex under the conditions used; however, Exo III does bind to the MutY.	bind
35156	2	10049	6	11	NULL	NULL	NULL	statement 1	GP		bind		cooperatively			cAMP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_21500_s_352	16728394	A distinct finding was that the PKA holoenzyme associated RI subunit-bound cAMP with positive cooperativity, because of intrachain interaction between the A and B sites.	bind
35157	3	10049	6	11	NULL	NULL	NULL				interacts with			A site					B site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_21500_s_352	16728394	A distinct finding was that the PKA holoenzyme associated RI subunit-bound cAMP with positive cooperativity, because of intrachain interaction between the A and B sites.	bind
49517	1	10049	6	11	NULL	NULL	NULL	RI subunit	GP		is associated with					PKA holoenzyme	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_21500_s_352	16728394	A distinct finding was that the PKA holoenzyme associated RI subunit-bound cAMP with positive cooperativity, because of intrachain interaction between the A and B sites.	bind
49518	4	10049	6	11	NULL	NULL	NULL	statement 3	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_21500_s_352	16728394	A distinct finding was that the PKA holoenzyme associated RI subunit-bound cAMP with positive cooperativity, because of intrachain interaction between the A and B sites.	bind
42878	1	10049	7	11	NULL	NULL	NULL	RI subunit	GP		is associated with					PKA holoenzyme	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_21500_s_352	16728394	A distinct finding was that the PKA holoenzyme associated RI subunit-bound cAMP with positive cooperativity, because of intrachain interaction between the A and B sites.	bind
42879	2	10049	7	11	NULL	NULL	NULL	statement 1	GP		bind		cooperatively			cAMP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_21500_s_352	16728394	A distinct finding was that the PKA holoenzyme associated RI subunit-bound cAMP with positive cooperativity, because of intrachain interaction between the A and B sites.	bind
42881	3	10049	7	11	NULL	NULL	NULL				interacts with			A site					B site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_21500_s_352	16728394	A distinct finding was that the PKA holoenzyme associated RI subunit-bound cAMP with positive cooperativity, because of intrachain interaction between the A and B sites.	bind
42882	4	10049	7	11	NULL	NULL	NULL	statement 3	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_21500_s_352	16728394	A distinct finding was that the PKA holoenzyme associated RI subunit-bound cAMP with positive cooperativity, because of intrachain interaction between the A and B sites.	bind
35158	1	10050	6	11	NULL	NULL	NULL	Mac-1 positive cells	Cell		bind		specifically			G-CSF	GP				NULL	peripheral blood of mice	NULL	NULL	NULL	NULL	gw60_jclininvest_102_3_483_s_139	9691084	A distinct Mac-1 positive population of  cells that specifically bound G-CSF was detected in the peripheral blood of mice of each genotype (Fig.  2 B); the slight increase in G-CSF binding seen with Wt/Mt or Mt/Mt cells was a  consistent finding.	bind
35159	2	10050	6	11	NULL	NULL	NULL	G-CSF	GP	binding of	increased in					Wt/Mt cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_3_483_s_139	9691084	A distinct Mac-1 positive population of  cells that specifically bound G-CSF was detected in the peripheral blood of mice of each genotype (Fig.  2 B); the slight increase in G-CSF binding seen with Wt/Mt or Mt/Mt cells was a  consistent finding.	bind
35160	3	10050	6	11	NULL	NULL	NULL	G-CSF	GP	binding of	is increased in					Mt/Mt cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_3_483_s_139	9691084	A distinct Mac-1 positive population of  cells that specifically bound G-CSF was detected in the peripheral blood of mice of each genotype (Fig.  2 B); the slight increase in G-CSF binding seen with Wt/Mt or Mt/Mt cells was a  consistent finding.	bind
42883	1	10050	7	11	NULL	NULL	NULL	Mac-1 positive cells	Cell		bind		specifically			G-CSF	GP				NULL	peripheral blood of mice 	NULL	NULL	NULL	NULL	gw60_jclininvest_102_3_483_s_139	9691084	A distinct Mac-1 positive population of  cells that specifically bound G-CSF was detected in the peripheral blood of mice of each genotype (Fig.  2 B); the slight increase in G-CSF binding seen with Wt/Mt or Mt/Mt cells was a  consistent finding.	bind
42897	2	10050	7	11	NULL	NULL	NULL	G-CSF	GP	binding of	increased in					Wt/Mt cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_3_483_s_139	9691084	A distinct Mac-1 positive population of  cells that specifically bound G-CSF was detected in the peripheral blood of mice of each genotype (Fig.  2 B); the slight increase in G-CSF binding seen with Wt/Mt or Mt/Mt cells was a  consistent finding.	bind
42898	3	10050	7	11	NULL	NULL	NULL	G-CSF	GP	binding of	increased in					Mt/Mt cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_3_483_s_139	9691084	A distinct Mac-1 positive population of  cells that specifically bound G-CSF was detected in the peripheral blood of mice of each genotype (Fig.  2 B); the slight increase in G-CSF binding seen with Wt/Mt or Mt/Mt cells was a  consistent finding.	bind
35161	1	10051	6	11	NULL	NULL	NULL	transcription factor	GP	distinct negative	bind		may							GT elements	NULL	root cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_51_32593_s_83	8955086	A distinct negative transcription factor may bind to GT elements, resulting in transcription repression in root cells.	bind
35162	2	10051	6	11	NULL	NULL	NULL	statement 1	Process		results in					transcription	Process	repression of			NULL	root cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_51_32593_s_83	8955086	A distinct negative transcription factor may bind to GT elements, resulting in transcription repression in root cells.	bind
42899	1	10051	7	11	NULL	NULL	NULL	transcription factor	GP	distinct negative	bind		may							GT elements	NULL	root cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_51_32593_s_83	8955086	A distinct negative transcription factor may bind to GT elements, resulting in transcription repression in root cells.	bind
42900	2	10051	7	11	NULL	NULL	NULL	statement 1	Process		results in					transcription	Process	repression of			NULL	root cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_51_32593_s_83	8955086	A distinct negative transcription factor may bind to GT elements, resulting in transcription repression in root cells.	bind
35163	1	10052	6	11	NULL	NULL	NULL	PKG-I	GP		bind			NH2-terminal leucine-zipper domain		MYPT1	GP		COOH-terminal leucine-zipper domain		NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_68_0_345_s_361	16460276	A distinct PKG-specific mechanism  involves binding of the NH2-terminal leucine-zipper domain of PKG-I  to the COOH-terminal leucine-zipper domain  of MYPT1.	bind
49519	2	10052	6	11	NULL	NULL	NULL	PKG-specific mechanism	GP		involves					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_68_0_345_s_361	16460276	A distinct PKG-specific mechanism  involves binding of the NH2-terminal leucine-zipper domain of PKG-I  to the COOH-terminal leucine-zipper domain  of MYPT1.	bind
42901	1	10052	7	11	NULL	NULL	NULL	PKG-I	GP		binds to			NH2-terminal leucine-zipper domain		MYPT1	GP		COOH-terminal leucine-zipper domain		NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_68_0_345_s_361	16460276	A distinct PKG-specific mechanism  involves binding of the NH2-terminal leucine-zipper domain of PKG-I  to the COOH-terminal leucine-zipper domain  of MYPT1.	bind
42902	2	10052	7	11	NULL	NULL	NULL	PKG-specific mechanism	GP		involves					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_68_0_345_s_361	16460276	A distinct PKG-specific mechanism  involves binding of the NH2-terminal leucine-zipper domain of PKG-I  to the COOH-terminal leucine-zipper domain  of MYPT1.	bind
35164	1	10053	6	11	NULL	NULL	NULL	GRH	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_gene_307_0_77_s_30	12706890	A distinct regulatory element, the upstream regulatory element (URE), is bound by the Grainyhead (GRH) transcription factor (   Hayashi et al., 1999).	bind
35165	2	10053	6	11	NULL	NULL	NULL	GRH	GP		is					Grainyhead	GP				NULL		NULL	NULL	NULL	NULL	gw60_gene_307_0_77_s_30	12706890	A distinct regulatory element, the upstream regulatory element (URE), is bound by the Grainyhead (GRH) transcription factor (   Hayashi et al., 1999).	bind
35166	3	10053	6	11	NULL	NULL	NULL	GRH	GP		bind									URE	NULL		NULL	NULL	NULL	NULL	gw60_gene_307_0_77_s_30	12706890	A distinct regulatory element, the upstream regulatory element (URE), is bound by the Grainyhead (GRH) transcription factor (   Hayashi et al., 1999).	bind
35167	4	10053	6	11	NULL	NULL	NULL	URE	NucleicAcid		is					upstream regulatory element	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_gene_307_0_77_s_30	12706890	A distinct regulatory element, the upstream regulatory element (URE), is bound by the Grainyhead (GRH) transcription factor (   Hayashi et al., 1999).	bind
42903	1	10053	7	11	NULL	NULL	NULL	GRH	GP		bind									URE	NULL		NULL	NULL	NULL	NULL	gw60_gene_307_0_77_s_30	12706890	A distinct regulatory element, the upstream regulatory element (URE), is bound by the Grainyhead (GRH) transcription factor (   Hayashi et al., 1999).	bind
42904	2	10053	7	11	NULL	NULL	NULL	GRH	GP		is					Grainyhead	GP				NULL		NULL	NULL	NULL	NULL	gw60_gene_307_0_77_s_30	12706890	A distinct regulatory element, the upstream regulatory element (URE), is bound by the Grainyhead (GRH) transcription factor (   Hayashi et al., 1999).	bind
42905	3	10053	7	11	NULL	NULL	NULL	URE	NucleicAcid		is					upstream regulatory element	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_gene_307_0_77_s_30	12706890	A distinct regulatory element, the upstream regulatory element (URE), is bound by the Grainyhead (GRH) transcription factor (   Hayashi et al., 1999).	bind
49520	4	10053	7	11	NULL	NULL	NULL	GRH	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_gene_307_0_77_s_30	12706890	A distinct regulatory element, the upstream regulatory element (URE), is bound by the Grainyhead (GRH) transcription factor (   Hayashi et al., 1999).	bind
35168	1	10054	6	11	NULL	NULL	NULL	GLD-3	GP		bind					GLD-2	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_101_13_4407_s_42	15070731	A distinct RNA-binding protein, GLD-3 ( ), binds to GLD-2 and stimulates its polyadenylation activity  in vitro ( ).	bind
35169	2	10054	6	11	NULL	NULL	NULL	GLD-3	GP		is a type of					RNA-binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_13_4407_s_42	15070731	A distinct RNA-binding protein, GLD-3 ( ), binds to GLD-2 and stimulates its polyadenylation activity  in vitro ( ).	bind
35170	3	10054	6	11	NULL	NULL	NULL	statement 1	Process		stimulates					GLD-2	GP	polyadenylation activity of			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_101_13_4407_s_42	15070731	A distinct RNA-binding protein, GLD-3 ( ), binds to GLD-2 and stimulates its polyadenylation activity  in vitro ( ).	bind
42906	1	10054	7	11	NULL	NULL	NULL	GLD-3 	GP		binds to					GLD-2	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_101_13_4407_s_42	15070731	A distinct RNA-binding protein, GLD-3 ( ), binds to GLD-2 and stimulates its polyadenylation activity  in vitro ( ).	bind
42907	2	10054	7	11	NULL	NULL	NULL	statement 1	Process		stimulates					GLD-2	GP	polyadenylation activity of			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_101_13_4407_s_42	15070731	A distinct RNA-binding protein, GLD-3 ( ), binds to GLD-2 and stimulates its polyadenylation activity  in vitro ( ).	bind
42908	3	10054	7	11	NULL	NULL	NULL	GLD-3 	GP		is a type of					RNA-binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_13_4407_s_42	15070731	A distinct RNA-binding protein, GLD-3 ( ), binds to GLD-2 and stimulates its polyadenylation activity  in vitro ( ).	bind
35171	1	10055	6	11	NULL	NULL	NULL	Grb2	GP		bind		constitutively			HPK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_44_27804_s_203	9346925	A distinction between Grb2 and Nck binding to HPK1 is that the interaction of HPK1 with Grb2 appears constitutive, whereas its association with Nck is stimulated by EGF stimulation (Figs.  5 A and  6).	bind
35172	2	10055	6	11	NULL	NULL	NULL	Nck	GP		bind					HPK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_44_27804_s_203	9346925	A distinction between Grb2 and Nck binding to HPK1 is that the interaction of HPK1 with Grb2 appears constitutive, whereas its association with Nck is stimulated by EGF stimulation (Figs.  5 A and  6).	bind
35173	3	10055	6	11	NULL	NULL	NULL	statement 2	Process		is stimulated by					EGF	GP	stimulation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_44_27804_s_203	9346925	A distinction between Grb2 and Nck binding to HPK1 is that the interaction of HPK1 with Grb2 appears constitutive, whereas its association with Nck is stimulated by EGF stimulation (Figs.  5 A and  6).	bind
42909	1	10055	7	11	NULL	NULL	NULL	Grb2	GP		binds		constitutively			HPK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_44_27804_s_203	9346925	A distinction between Grb2 and Nck binding to HPK1 is that the interaction of HPK1 with Grb2 appears constitutive, whereas its association with Nck is stimulated by EGF stimulation (Figs.  5 A and  6).	bind
42910	2	10055	7	11	NULL	NULL	NULL	Nck	GP		binds					HPK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_44_27804_s_203	9346925	A distinction between Grb2 and Nck binding to HPK1 is that the interaction of HPK1 with Grb2 appears constitutive, whereas its association with Nck is stimulated by EGF stimulation (Figs.  5 A and  6).	bind
42912	3	10055	7	11	NULL	NULL	NULL	EGF	GP	stimulation of	stimulates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_44_27804_s_203	9346925	A distinction between Grb2 and Nck binding to HPK1 is that the interaction of HPK1 with Grb2 appears constitutive, whereas its association with Nck is stimulated by EGF stimulation (Figs.  5 A and  6).	bind
35174	1	10056	6	11	NULL	NULL	NULL	IGFBP-6	GP		bind		high affinity			IGF-II	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14587_s_214	10329650	A distinctive feature of IGFBP-6 compared with IGFBPs 1-5 is its high binding affinity for IGF-II and its marked preferential binding of IGF-II relative to IGF-I.	bind
49558	2	10056	6	11	NULL	NULL	NULL	IGFBP-6	GP		bind					IGF-I	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14587_s_214	10329650	A distinctive feature of IGFBP-6 compared with IGFBPs 1-5 is its high binding affinity for IGF-II and its marked preferential binding of IGF-II relative to IGF-I.	bind
49559	3	10056	6	11	NULL	NULL	NULL	statement 1	Process		is more preferential than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14587_s_214	10329650	A distinctive feature of IGFBP-6 compared with IGFBPs 1-5 is its high binding affinity for IGF-II and its marked preferential binding of IGF-II relative to IGF-I.	bind
42913	1	10056	7	11	NULL	NULL	NULL	IGFBP-6	GP		bind		high affinity			IGF-II	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14587_s_214	10329650	A distinctive feature of IGFBP-6 compared with IGFBPs 1-5 is its high binding affinity for IGF-II and its marked preferential binding of IGF-II relative to IGF-I.	bind
42914	2	10056	7	11	NULL	NULL	NULL	IGFBP-6	GP		bind					IGF-I	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14587_s_214	10329650	A distinctive feature of IGFBP-6 compared with IGFBPs 1-5 is its high binding affinity for IGF-II and its marked preferential binding of IGF-II relative to IGF-I.	bind
42915	3	10056	7	11	NULL	NULL	NULL	statement 1	Process		is preferred over					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14587_s_214	10329650	A distinctive feature of IGFBP-6 compared with IGFBPs 1-5 is its high binding affinity for IGF-II and its marked preferential binding of IGF-II relative to IGF-I.	bind
42916	4	10056	7	11	NULL	NULL	NULL	IGFBP-1	GP		bind					IGF-II	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14587_s_214	10329650	A distinctive feature of IGFBP-6 compared with IGFBPs 1-5 is its high binding affinity for IGF-II and its marked preferential binding of IGF-II relative to IGF-I.	bind
42917	5	10056	7	11	NULL	NULL	NULL	IGFBP-2	GP		bind					IGF-II	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14587_s_214	10329650	A distinctive feature of IGFBP-6 compared with IGFBPs 1-5 is its high binding affinity for IGF-II and its marked preferential binding of IGF-II relative to IGF-I.	bind
42918	6	10056	7	11	NULL	NULL	NULL	IGFBP-3	GP		bind					IGF-II	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14587_s_214	10329650	A distinctive feature of IGFBP-6 compared with IGFBPs 1-5 is its high binding affinity for IGF-II and its marked preferential binding of IGF-II relative to IGF-I.	bind
42919	7	10056	7	11	NULL	NULL	NULL	IGFBP-4	GP		bind					IGF-II	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14587_s_214	10329650	A distinctive feature of IGFBP-6 compared with IGFBPs 1-5 is its high binding affinity for IGF-II and its marked preferential binding of IGF-II relative to IGF-I.	bind
42920	8	10056	7	11	NULL	NULL	NULL	IGFBP-5	GP		bind					IGF-II	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14587_s_214	10329650	A distinctive feature of IGFBP-6 compared with IGFBPs 1-5 is its high binding affinity for IGF-II and its marked preferential binding of IGF-II relative to IGF-I.	bind
42921	9	10056	7	11	NULL	NULL	NULL	statement 1	Process	binding affinity of	is higher than					statement 4	Process	binding affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14587_s_214	10329650	A distinctive feature of IGFBP-6 compared with IGFBPs 1-5 is its high binding affinity for IGF-II and its marked preferential binding of IGF-II relative to IGF-I.	bind
42922	10	10056	7	11	NULL	NULL	NULL	statement 1	Process	binding affinity of	is higher than					statement 5	Process	binding affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14587_s_214	10329650	A distinctive feature of IGFBP-6 compared with IGFBPs 1-5 is its high binding affinity for IGF-II and its marked preferential binding of IGF-II relative to IGF-I.	bind
42923	11	10056	7	11	NULL	NULL	NULL	statement 1	Process	binding affinity of	is higher than					statement 6	Process	binding affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14587_s_214	10329650	A distinctive feature of IGFBP-6 compared with IGFBPs 1-5 is its high binding affinity for IGF-II and its marked preferential binding of IGF-II relative to IGF-I.	bind
42924	12	10056	7	11	NULL	NULL	NULL	statement 1	Process	binding affinity of	is higher than					statement 7	Process	binding affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14587_s_214	10329650	A distinctive feature of IGFBP-6 compared with IGFBPs 1-5 is its high binding affinity for IGF-II and its marked preferential binding of IGF-II relative to IGF-I.	bind
42925	13	10056	7	11	NULL	NULL	NULL	statement 1	Process	binding affinity of	is higher than					statement 8	Process	binding affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14587_s_214	10329650	A distinctive feature of IGFBP-6 compared with IGFBPs 1-5 is its high binding affinity for IGF-II and its marked preferential binding of IGF-II relative to IGF-I.	bind
35175	1	10057	6	11	NULL	NULL	NULL	RdgC	GP		bind					plasmid DNA	NucleicAcid	circular			NULL		NULL	NULL	NULL	NULL	gw70_embo_22_3_735_s_75	12554673	A distributive mode of binding is also supported by the fact that  RdgC binds circular plasmid DNA and uniformly protects linear duplex DNA from attack  by hydroxyl radicals (data not shown).	bind
35176	2	10057	6	11	NULL	NULL	NULL	hydroxyl radicals	Chemical		attack					duplex DNA	NucleicAcid	linear			NULL		NULL	NULL	NULL	NULL	gw70_embo_22_3_735_s_75	12554673	A distributive mode of binding is also supported by the fact that  RdgC binds circular plasmid DNA and uniformly protects linear duplex DNA from attack  by hydroxyl radicals (data not shown).	bind
35177	3	10057	6	11	NULL	NULL	NULL	statement 1	Process		protects		uniformly			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_22_3_735_s_75	12554673	A distributive mode of binding is also supported by the fact that  RdgC binds circular plasmid DNA and uniformly protects linear duplex DNA from attack  by hydroxyl radicals (data not shown).	bind
42926	1	10057	7	11	NULL	NULL	NULL	 RdgC 	GP		binds					plasmid DNA	NucleicAcid	circular			NULL		NULL	NULL	NULL	NULL	gw70_embo_22_3_735_s_75	12554673	A distributive mode of binding is also supported by the fact that  RdgC binds circular plasmid DNA and uniformly protects linear duplex DNA from attack  by hydroxyl radicals (data not shown).	bind
42927	2	10057	7	11	NULL	NULL	NULL	hydroxyl radicals	Chemical		attack					duplex DNA	NucleicAcid	linear			NULL		NULL	NULL	NULL	NULL	gw70_embo_22_3_735_s_75	12554673	A distributive mode of binding is also supported by the fact that  RdgC binds circular plasmid DNA and uniformly protects linear duplex DNA from attack  by hydroxyl radicals (data not shown).	bind
42928	3	10057	7	11	NULL	NULL	NULL	statement 1	Process		protects		uniformly			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_22_3_735_s_75	12554673	A distributive mode of binding is also supported by the fact that  RdgC binds circular plasmid DNA and uniformly protects linear duplex DNA from attack  by hydroxyl radicals (data not shown).	bind
35183	1	10059	6	11	NULL	NULL	NULL	AP20187	Chemical		is a type of					divalent Fv ligand	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_19_16466_s_67	12637514	A divalent Fv ligand, AP20187, binds to Fv with high affinity but not to endogenous FKBP, thus minimizing the interference from endogenous FKBP and allowing for the effective dimerization of Fv fusion proteins.	bind
35184	2	10059	6	11	NULL	NULL	NULL	AP20187	Chemical		bind		high affinity			Fv	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_19_16466_s_67	12637514	A divalent Fv ligand, AP20187, binds to Fv with high affinity but not to endogenous FKBP, thus minimizing the interference from endogenous FKBP and allowing for the effective dimerization of Fv fusion proteins.	bind
35186	3	10059	6	11	NULL	NULL	NULL	AP20187	Chemical		does not bind					FKBP	GP	endogenous			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_19_16466_s_67	12637514	A divalent Fv ligand, AP20187, binds to Fv with high affinity but not to endogenous FKBP, thus minimizing the interference from endogenous FKBP and allowing for the effective dimerization of Fv fusion proteins.	bind
35602	4	10059	6	11	NULL	NULL	NULL	statement 2	Process		allows					Fv fusion proteins	GP	effective;;dimerization of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_19_16466_s_67	12637514	A divalent Fv ligand, AP20187, binds to Fv with high affinity but not to endogenous FKBP, thus minimizing the interference from endogenous FKBP and allowing for the effective dimerization of Fv fusion proteins.	bind
49521	5	10059	6	11	NULL	NULL	NULL	statement 2	Process		minimize					FKBP	GP	interference from;;endogenous			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_19_16466_s_67	12637514	A divalent Fv ligand, AP20187, binds to Fv with high affinity but not to endogenous FKBP, thus minimizing the interference from endogenous FKBP and allowing for the effective dimerization of Fv fusion proteins.	bind
42929	1	10059	7	11	NULL	NULL	NULL	AP20187	Chemical		binds to		high affinity			Fv	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_19_16466_s_67	12637514	A divalent Fv ligand, AP20187, binds to Fv with high affinity but not to endogenous FKBP, thus minimizing the interference from endogenous FKBP and allowing for the effective dimerization of Fv fusion proteins.	bind
42930	2	10059	7	11	NULL	NULL	NULL	AP20187	Chemical		does not bind					FKBP	GP	endogenous			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_19_16466_s_67	12637514	A divalent Fv ligand, AP20187, binds to Fv with high affinity but not to endogenous FKBP, thus minimizing the interference from endogenous FKBP and allowing for the effective dimerization of Fv fusion proteins.	bind
42931	3	10059	7	11	NULL	NULL	NULL	statement 1	Process		minimize					 FKBP	GP	interference from;;endogenous			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_19_16466_s_67	12637514	A divalent Fv ligand, AP20187, binds to Fv with high affinity but not to endogenous FKBP, thus minimizing the interference from endogenous FKBP and allowing for the effective dimerization of Fv fusion proteins.	bind
42932	4	10059	7	11	NULL	NULL	NULL	statement 1	Process		allows					Fv fusion proteins	GP	effective;;dimerization of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_19_16466_s_67	12637514	A divalent Fv ligand, AP20187, binds to Fv with high affinity but not to endogenous FKBP, thus minimizing the interference from endogenous FKBP and allowing for the effective dimerization of Fv fusion proteins.	bind
57267	5	10059	7	11	NULL	NULL	NULL	AP20187	Process		is a type of					divalent Fv ligand	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_19_16466_s_67	12637514	A divalent Fv ligand, AP20187, binds to Fv with high affinity but not to endogenous FKBP, thus minimizing the interference from endogenous FKBP and allowing for the effective dimerization of Fv fusion proteins.	bind
35190	1	10060	6	11	NULL	NULL	NULL	IL-6	GP		induces					STAT3-LUC	GP	expression of			NULL	293T cells	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_315_3_692_s_68	14975756	A DN-STAT3 significantly inhibited IL-6- or LIF-induced STAT3-LUC expression in  a dose-dependent fashion in 293T cells as described previously [ 27].	bind
35191	2	10060	6	11	NULL	NULL	NULL	LIF	GP		induces					STAT3-LUC	GP	expression of			NULL	293T cells	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_315_3_692_s_68	14975756	A DN-STAT3 significantly inhibited IL-6- or LIF-induced STAT3-LUC expression in  a dose-dependent fashion in 293T cells as described previously [ 27].	bind
35194	3	10060	6	11	NULL	NULL	NULL	DN-STAT3	GP		inhibits		significantly;;dose dependently			statement 1	Process				NULL	293T cells	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_315_3_692_s_68	14975756	A DN-STAT3 significantly inhibited IL-6- or LIF-induced STAT3-LUC expression in  a dose-dependent fashion in 293T cells as described previously [ 27].	bind
35195	4	10060	6	11	NULL	NULL	NULL	DN-STAT3	GP		inhibits		significantly;;dose dependently			statement 2	Process				NULL	293T cells	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_315_3_692_s_68	14975756	A DN-STAT3 significantly inhibited IL-6- or LIF-induced STAT3-LUC expression in  a dose-dependent fashion in 293T cells as described previously [ 27].	bind
42933	3	10060	7	11	NULL	NULL	NULL	DN-STAT3	GP		inhibits		significantly;;dose dependently			statement 1	Process				NULL	293T cells	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_315_3_692_s_68	14975756	A DN-STAT3 significantly inhibited IL-6- or LIF-induced STAT3-LUC expression in  a dose-dependent fashion in 293T cells as described previously [ 27].	bind
42934	2	10060	7	11	NULL	NULL	NULL	LIF	GP		induce					 STAT3-LUC	GP	expression of			NULL	293T cells	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_315_3_692_s_68	14975756	A DN-STAT3 significantly inhibited IL-6- or LIF-induced STAT3-LUC expression in  a dose-dependent fashion in 293T cells as described previously [ 27].	bind
42935	4	10060	7	11	NULL	NULL	NULL	DN-STAT3	GP		inhibits		significantly;;dose dependently			statement 2	Process				NULL	293T cells	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_315_3_692_s_68	14975756	A DN-STAT3 significantly inhibited IL-6- or LIF-induced STAT3-LUC expression in  a dose-dependent fashion in 293T cells as described previously [ 27].	bind
49522	1	10060	7	11	NULL	NULL	NULL	IL-6	GP		induces					STAT3-LUC	GP	expression of			NULL	293T cells	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_315_3_692_s_68	14975756	A DN-STAT3 significantly inhibited IL-6- or LIF-induced STAT3-LUC expression in  a dose-dependent fashion in 293T cells as described previously [ 27].	bind
35603	3	10061	6	11	NULL	NULL	NULL	statement 1	Chemical		bind		cooperatively							CD28RE-TRE Sequence	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_1_552_s_110	9417115	A DNA Affinity-purified Multicomponent Complex from Ionomycin/PMA-and Anti-CD28 mAb-stimulated Jurkat T-cells Binds Cooperatively to the CD28RE-TRE Sequence-- A DNA-binding protein complex was isolated from ionomycin/PMA/anti-CD28 mAb-stimulated Jurkat T-cells by DNA affinity chromatography (Fig.  2).	bind
35604	4	10061	6	11	NULL	NULL	NULL	statement 2	GP		bind		cooperatively							CD28RE-TRE Sequence	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_1_552_s_110	9417115	A DNA Affinity-purified Multicomponent Complex from Ionomycin/PMA-and Anti-CD28 mAb-stimulated Jurkat T-cells Binds Cooperatively to the CD28RE-TRE Sequence-- A DNA-binding protein complex was isolated from ionomycin/PMA/anti-CD28 mAb-stimulated Jurkat T-cells by DNA affinity chromatography (Fig.  2).	bind
57317	1	10061	6	11	NULL	NULL	NULL	Ionomycin/PMA	Chemical		stimulates					Jurkat T-cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_1_552_s_110	9417115	A DNA Affinity-purified Multicomponent Complex from Ionomycin/PMA-and Anti-CD28 mAb-stimulated Jurkat T-cells Binds Cooperatively to the CD28RE-TRE Sequence-- A DNA-binding protein complex was isolated from ionomycin/PMA/anti-CD28 mAb-stimulated Jurkat T-cells by DNA affinity chromatography (Fig.  2).	bind
57318	2	10061	6	11	NULL	NULL	NULL	Anti-CD28 mAb	GP		stimulates					Jurkat T-cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_1_552_s_110	9417115	A DNA Affinity-purified Multicomponent Complex from Ionomycin/PMA-and Anti-CD28 mAb-stimulated Jurkat T-cells Binds Cooperatively to the CD28RE-TRE Sequence-- A DNA-binding protein complex was isolated from ionomycin/PMA/anti-CD28 mAb-stimulated Jurkat T-cells by DNA affinity chromatography (Fig.  2).	bind
42936	1	10061	7	11	NULL	NULL	NULL	Ionomycin/PMA mAb	GP		stimulate					Jurkat T-cells 	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_1_552_s_110	9417115	A DNA Affinity-purified Multicomponent Complex from Ionomycin/PMA-and Anti-CD28 mAb-stimulated Jurkat T-cells Binds Cooperatively to the CD28RE-TRE Sequence-- A DNA-binding protein complex was isolated from ionomycin/PMA/anti-CD28 mAb-stimulated Jurkat T-cells by DNA affinity chromatography (Fig.  2).	bind
42937	2	10061	7	11	NULL	NULL	NULL	Anti-CD28 mAb	GP		stimulate					Jurkat T-cells 	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_1_552_s_110	9417115	A DNA Affinity-purified Multicomponent Complex from Ionomycin/PMA-and Anti-CD28 mAb-stimulated Jurkat T-cells Binds Cooperatively to the CD28RE-TRE Sequence-- A DNA-binding protein complex was isolated from ionomycin/PMA/anti-CD28 mAb-stimulated Jurkat T-cells by DNA affinity chromatography (Fig.  2).	bind
42938	3	10061	7	11	NULL	NULL	NULL	statement 1	Chemical		bind		cooperatively							CD28RE-TRE Sequence	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_1_552_s_110	9417115	A DNA Affinity-purified Multicomponent Complex from Ionomycin/PMA-and Anti-CD28 mAb-stimulated Jurkat T-cells Binds Cooperatively to the CD28RE-TRE Sequence-- A DNA-binding protein complex was isolated from ionomycin/PMA/anti-CD28 mAb-stimulated Jurkat T-cells by DNA affinity chromatography (Fig.  2).	bind
42939	4	10061	7	11	NULL	NULL	NULL	statement 2	GP		bind		cooperatively							CD28RE-TRE Sequence	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_1_552_s_110	9417115	A DNA Affinity-purified Multicomponent Complex from Ionomycin/PMA-and Anti-CD28 mAb-stimulated Jurkat T-cells Binds Cooperatively to the CD28RE-TRE Sequence-- A DNA-binding protein complex was isolated from ionomycin/PMA/anti-CD28 mAb-stimulated Jurkat T-cells by DNA affinity chromatography (Fig.  2).	bind
35198	1	10062	6	11	NULL	NULL	NULL	AP-1	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_63_3_607_s_178	12606768	A DNA binding activity of AP-1 and SP-1 was determined by gel mobility shift assay as described under  Materials and Methods.	bind
35199	2	10062	6	11	NULL	NULL	NULL	SP-1	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_63_3_607_s_178	12606768	A DNA binding activity of AP-1 and SP-1 was determined by gel mobility shift assay as described under  Materials and Methods.	bind
42940	1	10062	7	11	NULL	NULL	NULL	AP-1	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_63_3_607_s_178	12606768	A DNA binding activity of AP-1 and SP-1 was determined by gel mobility shift assay as described under  Materials and Methods.	bind
42941	2	10062	7	11	NULL	NULL	NULL	SP-1	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_63_3_607_s_178	12606768	A DNA binding activity of AP-1 and SP-1 was determined by gel mobility shift assay as described under  Materials and Methods.	bind
35205	1	10064	6	11	NULL	NULL	NULL	sod	GP	B. fragilis	bind		could		promoter	OxyR protein	GP	P. gingivalis			NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_microbiology_152_pt-4_16549660_s_11	16549660	A DNA fragment  including the B. fragilis sod promoter region could bind the P. gingivalis  OxyR protein; however, a putative OxyR binding sequence within the DNA  fragment was 14 bases distant from a putative -35 box of its promoter.	bind
42944	1	10064	7	11	NULL	NULL	NULL	sod	GP	B. fragilis	bind		could		promoter	OxyR protein	GP	P. gingivalis			NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_microbiology_152_pt-4_16549660_s_11	16549660	A DNA fragment  including the B. fragilis sod promoter region could bind the P. gingivalis  OxyR protein; however, a putative OxyR binding sequence within the DNA  fragment was 14 bases distant from a putative -35 box of its promoter.	bind
42945	2	10064	7	11	NULL	NULL	NULL	OxyR	GP		is present at				putative binding sequence within the DNA fragment	OxyR	GP			14 bases distant from a putative -35 box of promoter	NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_microbiology_152_pt-4_16549660_s_11	16549660	A DNA fragment  including the B. fragilis sod promoter region could bind the P. gingivalis  OxyR protein; however, a putative OxyR binding sequence within the DNA  fragment was 14 bases distant from a putative -35 box of its promoter.	bind
35605	1	10067	6	11	NULL	NULL	NULL	tissue-type plasminogen activator gene	GP	human	cooperate in				cAMP-responsive element of promoter	basal expression	Process				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_94_1_79_s_515	10842061	A DNA motif related to the cAMP-responsive element and an exon- located activator protein-2 binding site in the human tissue-type plasminogen activator gene promoter cooperate in basal expression and convey activation by phorbol ester and cAMP.	bind
35606	2	10067	6	11	NULL	NULL	NULL	tissue-type plasminogen activator gene	GP	human	cooperate in				exon- located activator protein-2 binding site of promoter	basal expression	Process				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_94_1_79_s_515	10842061	A DNA motif related to the cAMP-responsive element and an exon- located activator protein-2 binding site in the human tissue-type plasminogen activator gene promoter cooperate in basal expression and convey activation by phorbol ester and cAMP.	bind
35607	3	10067	6	11	NULL	NULL	NULL	tissue-type plasminogen activator gene	GP	human	is activated by				cAMP-responsive element of promoter	phorbol ester	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_94_1_79_s_515	10842061	A DNA motif related to the cAMP-responsive element and an exon- located activator protein-2 binding site in the human tissue-type plasminogen activator gene promoter cooperate in basal expression and convey activation by phorbol ester and cAMP.	bind
35608	4	10067	6	11	NULL	NULL	NULL	tissue-type plasminogen activator gene	GP	human	is activated by				cAMP-responsive element of promoter	cAMP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_94_1_79_s_515	10842061	A DNA motif related to the cAMP-responsive element and an exon- located activator protein-2 binding site in the human tissue-type plasminogen activator gene promoter cooperate in basal expression and convey activation by phorbol ester and cAMP.	bind
35609	5	10067	6	11	NULL	NULL	NULL	tissue-type plasminogen activator gene	GP	human	is activated by				exon- located activator protein-2 binding site of promoter	phorbol ester	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_94_1_79_s_515	10842061	A DNA motif related to the cAMP-responsive element and an exon- located activator protein-2 binding site in the human tissue-type plasminogen activator gene promoter cooperate in basal expression and convey activation by phorbol ester and cAMP.	bind
35610	6	10067	6	11	NULL	NULL	NULL	tissue-type plasminogen activator gene	GP	human	is activated by				exon- located activator protein-2 binding site of promoter	cAMP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_94_1_79_s_515	10842061	A DNA motif related to the cAMP-responsive element and an exon- located activator protein-2 binding site in the human tissue-type plasminogen activator gene promoter cooperate in basal expression and convey activation by phorbol ester and cAMP.	bind
42946	1	10067	7	11	NULL	NULL	NULL	tissue-type plasminogen activator gene	GP	human	cooperate in				DNA motif related to the cAMP-responsive element in the promoter	basal expression	Process				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_94_1_79_s_515	10842061	A DNA motif related to the cAMP-responsive element and an exon- located activator protein-2 binding site in the human tissue-type plasminogen activator gene promoter cooperate in basal expression and convey activation by phorbol ester and cAMP.	bind
42947	2	10067	7	11	NULL	NULL	NULL	tissue-type plasminogen activator gene	GP	human	cooperate in				 exon- located activator protein-2 binding site in the promoter	basal expression	Process				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_94_1_79_s_515	10842061	A DNA motif related to the cAMP-responsive element and an exon- located activator protein-2 binding site in the human tissue-type plasminogen activator gene promoter cooperate in basal expression and convey activation by phorbol ester and cAMP.	bind
42948	3	10067	7	11	NULL	NULL	NULL	phorbol ester	Chemical		activates					tissue-type plasminogen activator gene	GP	 human		DNA motif related to the cAMP-responsive element in the promoter	NULL		NULL	NULL	NULL	NULL	gw60_mechdev_94_1_79_s_515	10842061	A DNA motif related to the cAMP-responsive element and an exon- located activator protein-2 binding site in the human tissue-type plasminogen activator gene promoter cooperate in basal expression and convey activation by phorbol ester and cAMP.	bind
42949	4	10067	7	11	NULL	NULL	NULL	phorbol ester	Chemical		activates					tissue-type plasminogen activator gene	GP	human		exon- located activator protein-2 binding site in the promoter	NULL		NULL	NULL	NULL	NULL	gw60_mechdev_94_1_79_s_515	10842061	A DNA motif related to the cAMP-responsive element and an exon- located activator protein-2 binding site in the human tissue-type plasminogen activator gene promoter cooperate in basal expression and convey activation by phorbol ester and cAMP.	bind
42950	5	10067	7	11	NULL	NULL	NULL	cAMP	Chemical		activates					tissue-type plasminogen activator gene	GP	human		DNA motif related to the cAMP-responsive element in the promoter	NULL		NULL	NULL	NULL	NULL	gw60_mechdev_94_1_79_s_515	10842061	A DNA motif related to the cAMP-responsive element and an exon- located activator protein-2 binding site in the human tissue-type plasminogen activator gene promoter cooperate in basal expression and convey activation by phorbol ester and cAMP.	bind
42951	6	10067	7	11	NULL	NULL	NULL	cAMP	Chemical		activates					tissue-type plasminogen activator gene	GP	human		exon- located activator protein-2 binding site	NULL		NULL	NULL	NULL	NULL	gw60_mechdev_94_1_79_s_515	10842061	A DNA motif related to the cAMP-responsive element and an exon- located activator protein-2 binding site in the human tissue-type plasminogen activator gene promoter cooperate in basal expression and convey activation by phorbol ester and cAMP.	bind
35212	1	10068	6	11	NULL	NULL	NULL	BMP-7	GP		does not activate					2GC(MUT)-luc	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_18544_s_171	14981086	A DNA pulldown assay was carried out to examine whether lack of activation of 2GC(MUT)-luc by BMP7 is caused by lack of Smad4 binding to GC-1, GC-2, GC-3, and GC-pal motifs ( Fig. 3 B).	bind
35213	2	10068	6	11	NULL	NULL	NULL	Smad4	GP		does not bind									GC-1	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_18544_s_171	14981086	A DNA pulldown assay was carried out to examine whether lack of activation of 2GC(MUT)-luc by BMP7 is caused by lack of Smad4 binding to GC-1, GC-2, GC-3, and GC-pal motifs ( Fig. 3 B).	bind
35214	3	10068	6	11	NULL	NULL	NULL	Smad4	GP		does not bind									GC-2	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_18544_s_171	14981086	A DNA pulldown assay was carried out to examine whether lack of activation of 2GC(MUT)-luc by BMP7 is caused by lack of Smad4 binding to GC-1, GC-2, GC-3, and GC-pal motifs ( Fig. 3 B).	bind
35215	4	10068	6	11	NULL	NULL	NULL	Smad4	GP		does not bind									GC-3	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_18544_s_171	14981086	A DNA pulldown assay was carried out to examine whether lack of activation of 2GC(MUT)-luc by BMP7 is caused by lack of Smad4 binding to GC-1, GC-2, GC-3, and GC-pal motifs ( Fig. 3 B).	bind
35216	5	10068	6	11	NULL	NULL	NULL	Smad4	GP		does not bind									GC-pal motif	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_18544_s_171	14981086	A DNA pulldown assay was carried out to examine whether lack of activation of 2GC(MUT)-luc by BMP7 is caused by lack of Smad4 binding to GC-1, GC-2, GC-3, and GC-pal motifs ( Fig. 3 B).	bind
42952	1	10068	7	11	NULL	NULL	NULL	Smad4 	GP		does not bind									GC-1 motifs	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_18544_s_171	14981086	A DNA pulldown assay was carried out to examine whether lack of activation of 2GC(MUT)-luc by BMP7 is caused by lack of Smad4 binding to GC-1, GC-2, GC-3, and GC-pal motifs ( Fig. 3 B).	bind
42953	2	10068	7	11	NULL	NULL	NULL	Smad4	GP		does not bind									GC-2 motifs	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_18544_s_171	14981086	A DNA pulldown assay was carried out to examine whether lack of activation of 2GC(MUT)-luc by BMP7 is caused by lack of Smad4 binding to GC-1, GC-2, GC-3, and GC-pal motifs ( Fig. 3 B).	bind
42954	3	10068	7	11	NULL	NULL	NULL	Smad4	GP		does not bind									GC-3 motifs	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_18544_s_171	14981086	A DNA pulldown assay was carried out to examine whether lack of activation of 2GC(MUT)-luc by BMP7 is caused by lack of Smad4 binding to GC-1, GC-2, GC-3, and GC-pal motifs ( Fig. 3 B).	bind
42955	4	10068	7	11	NULL	NULL	NULL	Smad4	GP		does not bind									GC-pal motifs	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_18544_s_171	14981086	A DNA pulldown assay was carried out to examine whether lack of activation of 2GC(MUT)-luc by BMP7 is caused by lack of Smad4 binding to GC-1, GC-2, GC-3, and GC-pal motifs ( Fig. 3 B).	bind
42956	5	10068	7	11	NULL	NULL	NULL	BMP7	GP		does not activate					 2GC(MUT)-luc	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_18544_s_171	14981086	A DNA pulldown assay was carried out to examine whether lack of activation of 2GC(MUT)-luc by BMP7 is caused by lack of Smad4 binding to GC-1, GC-2, GC-3, and GC-pal motifs ( Fig. 3 B).	bind
35217	1	10069	6	11	NULL	NULL	NULL	chromosome	Chromosome	DNA segment of;;E. coli	bind				replication terminus region	XerC	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_new-biol_3_8_1931824_s_6	1931824	A DNA segment (dif)  from the replication terminus region of the E. coli chromosome binds XerC  and acts as a substrate for XerC-mediated site-specific recombination  when inserted into multicopy plasmids.	bind
35218	2	10069	6	11	NULL	NULL	NULL	XerC	GP		mediates					recombination	Process	site-specific			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_new-biol_3_8_1931824_s_6	1931824	A DNA segment (dif)  from the replication terminus region of the E. coli chromosome binds XerC  and acts as a substrate for XerC-mediated site-specific recombination  when inserted into multicopy plasmids.	bind
35225	3	10069	6	11	NULL	NULL	NULL	chromosome	Chromosome	DNA segment of;;E. coli	acts as a substrate for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_new-biol_3_8_1931824_s_6	1931824	A DNA segment (dif)  from the replication terminus region of the E. coli chromosome binds XerC  and acts as a substrate for XerC-mediated site-specific recombination  when inserted into multicopy plasmids.	bind
35226	4	10069	6	11	NULL	NULL	NULL	statement 2	Process		occurs when inserted into					multicopy plasmids	NucleicAcid				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_new-biol_3_8_1931824_s_6	1931824	A DNA segment (dif)  from the replication terminus region of the E. coli chromosome binds XerC  and acts as a substrate for XerC-mediated site-specific recombination  when inserted into multicopy plasmids.	bind
42961	1	10069	7	11	NULL	NULL	NULL	chromosome	Chromosome	DNA segment of;;E. coli	binds				replication terminus region of 	XerC	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_new-biol_3_8_1931824_s_6	1931824	A DNA segment (dif)  from the replication terminus region of the E. coli chromosome binds XerC  and acts as a substrate for XerC-mediated site-specific recombination  when inserted into multicopy plasmids.	bind
42962	2	10069	7	11	NULL	NULL	NULL	XerC	GP		mediate					recombination	Process	site-specific			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_new-biol_3_8_1931824_s_6	1931824	A DNA segment (dif)  from the replication terminus region of the E. coli chromosome binds XerC  and acts as a substrate for XerC-mediated site-specific recombination  when inserted into multicopy plasmids.	bind
42963	3	10069	7	11	NULL	NULL	NULL	chromosome	Chromosome	DNA segment of;;E. coli	acts as a substrate for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_new-biol_3_8_1931824_s_6	1931824	A DNA segment (dif)  from the replication terminus region of the E. coli chromosome binds XerC  and acts as a substrate for XerC-mediated site-specific recombination  when inserted into multicopy plasmids.	bind
35227	1	10070	6	11	NULL	NULL	NULL	MOP3-MOP4 heterodimer	GP		bind					DNA	NucleicAcid			CACGTGA element	NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_proc-natl-acad-sci-u-s-a_95_10_9576906_s_4	9576906	A DNA selection protocol revealed  that the MOP3-MOP4 heterodimer bound a CACGTGA-containing DNA element.	bind
42964	1	10070	7	11	NULL	NULL	NULL	MOP3-MOP4 heterodimer	GP		bind					DNA	NucleicAcid			CACGTGA element	NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_proc-natl-acad-sci-u-s-a_95_10_9576906_s_4	9576906	A DNA selection protocol revealed  that the MOP3-MOP4 heterodimer bound a CACGTGA-containing DNA element.	bind
35228	1	10071	6	11	NULL	NULL	NULL	DNA-binding protein	GP	Candida albicans	bind							Saccharomyces cerevisiae		RPG box	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_17_5273_s_336	10464197	A DNA-binding protein from  Candida albicans that binds to the RPG box of  Saccharomyces cerevisiae and the telomeric repeat sequence of  C. albicans.	bind
35230	2	10071	6	11	NULL	NULL	NULL	DNA-binding protein	GP	Candida albicans	bind							C.albicans		telomeric repeat sequence	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_17_5273_s_336	10464197	A DNA-binding protein from  Candida albicans that binds to the RPG box of  Saccharomyces cerevisiae and the telomeric repeat sequence of  C. albicans.	bind
42965	1	10071	7	11	NULL	NULL	NULL	DNA-binding protein	GP	 Candida albicans	binds to							Saccharomyces cerevisiae		RPG box	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_17_5273_s_336	10464197	A DNA-binding protein from  Candida albicans that binds to the RPG box of  Saccharomyces cerevisiae and the telomeric repeat sequence of  C. albicans.	bind
42966	2	10071	7	11	NULL	NULL	NULL	DNA-binding protein	GP	Candida albicans	binds to							C. albicans		telomeric repeat sequence 	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_17_5273_s_336	10464197	A DNA-binding protein from  Candida albicans that binds to the RPG box of  Saccharomyces cerevisiae and the telomeric repeat sequence of  C. albicans.	bind
35611	1	10072	6	11	NULL	NULL	NULL	RAG1	GP		bind					RSS	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_5584_s_310	12488446	A DNA-induced Conformational Change in RAG1--  It has been proposed previously that RAG2 can induce a conformational change in RAG1  that facilitates binding of RAG1 to the RSS and perhaps also the appropriate folding of the RAG1 DDE active site ( ,  ,  ).	bind
35612	2	10072	6	11	NULL	NULL	NULL	RAG2	GP		induces					RAG1	GP	conformational change in			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_5584_s_310	12488446	A DNA-induced Conformational Change in RAG1--  It has been proposed previously that RAG2 can induce a conformational change in RAG1  that facilitates binding of RAG1 to the RSS and perhaps also the appropriate folding of the RAG1 DDE active site ( ,  ,  ).	bind
35613	3	10072	6	11	NULL	NULL	NULL	statement 2	Process		facilitates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_5584_s_310	12488446	A DNA-induced Conformational Change in RAG1--  It has been proposed previously that RAG2 can induce a conformational change in RAG1  that facilitates binding of RAG1 to the RSS and perhaps also the appropriate folding of the RAG1 DDE active site ( ,  ,  ).	bind
35614	4	10072	6	11	NULL	NULL	NULL	statement 2	Process		facilitates		perhaps			RAG1	GP	folding of	DDE active site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_5584_s_310	12488446	A DNA-induced Conformational Change in RAG1--  It has been proposed previously that RAG2 can induce a conformational change in RAG1  that facilitates binding of RAG1 to the RSS and perhaps also the appropriate folding of the RAG1 DDE active site ( ,  ,  ).	bind
49525	5	10072	6	11	NULL	NULL	NULL	DNA	NucleicAcid		induce					RAG1	GP	\tconformational change in 			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_5584_s_310	12488446	A DNA-induced Conformational Change in RAG1--  It has been proposed previously that RAG2 can induce a conformational change in RAG1  that facilitates binding of RAG1 to the RSS and perhaps also the appropriate folding of the RAG1 DDE active site ( ,  ,  ).	bind
42967	1	10072	7	11	NULL	NULL	NULL	RAG2	GP		induce					RAG1	GP	conformational change in 			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_5584_s_310	12488446	A DNA-induced Conformational Change in RAG1--  It has been proposed previously that RAG2 can induce a conformational change in RAG1  that facilitates binding of RAG1 to the RSS and perhaps also the appropriate folding of the RAG1 DDE active site ( ,  ,  ).	bind
42968	2	10072	7	11	NULL	NULL	NULL	RAG1	GP		bind					RSS	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_5584_s_310	12488446	A DNA-induced Conformational Change in RAG1--  It has been proposed previously that RAG2 can induce a conformational change in RAG1  that facilitates binding of RAG1 to the RSS and perhaps also the appropriate folding of the RAG1 DDE active site ( ,  ,  ).	bind
42969	3	10072	7	11	NULL	NULL	NULL	statement 1	Process		facilitate					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_5584_s_310	12488446	A DNA-induced Conformational Change in RAG1--  It has been proposed previously that RAG2 can induce a conformational change in RAG1  that facilitates binding of RAG1 to the RSS and perhaps also the appropriate folding of the RAG1 DDE active site ( ,  ,  ).	bind
42970	4	10072	7	11	NULL	NULL	NULL	statement 1	Process		facilitate					RAG1	GP	folding of	DDE active site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_5584_s_310	12488446	A DNA-induced Conformational Change in RAG1--  It has been proposed previously that RAG2 can induce a conformational change in RAG1  that facilitates binding of RAG1 to the RSS and perhaps also the appropriate folding of the RAG1 DDE active site ( ,  ,  ).	bind
42971	5	10072	7	11	NULL	NULL	NULL	DNA	NucleicAcid		induce					RAG1	GP	conformational change in			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_5584_s_310	12488446	A DNA-induced Conformational Change in RAG1--  It has been proposed previously that RAG2 can induce a conformational change in RAG1  that facilitates binding of RAG1 to the RSS and perhaps also the appropriate folding of the RAG1 DDE active site ( ,  ,  ).	bind
35259	1	10074	6	11	NULL	NULL	NULL	Sc/Da	GP		bind									E1	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_13_2036_s_123	9649507	A DNase footprint assay indicated that Sc/Da bound to E1, but not to the N box (not shown).	bind
35261	2	10074	6	11	NULL	NULL	NULL	Sc/Da	GP		does not bind									N box	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_13_2036_s_123	9649507	A DNase footprint assay indicated that Sc/Da bound to E1, but not to the N box (not shown).	bind
42972	1	10074	7	11	NULL	NULL	NULL	Sc/Da	GP		bind									E1	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_13_2036_s_123	9649507	A DNase footprint assay indicated that Sc/Da bound to E1, but not to the N box (not shown).	bind
42973	2	10074	7	11	NULL	NULL	NULL	Sc/Da	GP		does not bind									N box	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_13_2036_s_123	9649507	A DNase footprint assay indicated that Sc/Da bound to E1, but not to the N box (not shown).	bind
35263	1	10075	6	11	NULL	NULL	NULL	OmpR	GP		bind		may;; directly			ssrA	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_3_771_s_175	10633113	A DNase I protection assay was used to determine if OmpR binds directly to the  ssrA promoter region.	bind
42974	1	10075	7	11	NULL	NULL	NULL	OmpR	GP		binds		may;;directly			ssrA	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_3_771_s_175	10633113	A DNase I protection assay was used to determine if OmpR binds directly to the  ssrA promoter region.	bind
35269	1	10076	6	11	NULL	NULL	NULL	cullin	GP		bind		selectively	DOC domain		Skp1-Fbx29	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_47_43824_s_232	11568188	A DOC domain-containing cullin selectively binds Skp1{middle dot}Fbx29 to form an SCF-like complex          PNAS,                       December 24, 2002;  99(26):  16601 - 16606.	bind
36456	2	10076	6	11	NULL	NULL	NULL	statement 1	Process		forms					SCF-like complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_47_43824_s_232	11568188	A DOC domain-containing cullin selectively binds Skp1{middle dot}Fbx29 to form an SCF-like complex          PNAS,                       December 24, 2002;  99(26):  16601 - 16606.	bind
42982	1	10076	7	11	NULL	NULL	NULL	cullin	GP		binds		selectively	DOC domain		Skp1-Fbx29	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_47_43824_s_232	11568188	A DOC domain-containing cullin selectively binds Skp1{middle dot}Fbx29 to form an SCF-like complex          PNAS,                       December 24, 2002;  99(26):  16601 - 16606.	bind
42983	2	10076	7	11	NULL	NULL	NULL	statement 1	Process		forms					SCF-like complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_47_43824_s_232	11568188	A DOC domain-containing cullin selectively binds Skp1{middle dot}Fbx29 to form an SCF-like complex          PNAS,                       December 24, 2002;  99(26):  16601 - 16606.	bind
35274	1	10078	6	11	NULL	NULL	NULL	p130CAS	GP		bind			SH3 domain		FAK	GP		PR1		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_8_6802_s_319	15557280	A docking molecule p130CAS binds to PR1 of FAK through its SH3 domain ( ).	bind
42984	1	10078	7	11	NULL	NULL	NULL	p130CAS	GP		binds to			 SH3 domain		FAK	GP		PR1		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_8_6802_s_319	15557280	A docking molecule p130CAS binds to PR1 of FAK through its SH3 domain ( ).	bind
35275	1	10079	6	11	NULL	NULL	NULL	Ras-Rac pathway	GP		mediates					cell transformation	Process				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_3834	10066831	A domain containing the Cdc42/Rac interactive binding (CRIB) region of p65PAK inhibits transcriptional activation and cell transformation mediated by the Ras-Rac pathway.	bind
35276	2	10079	6	11	NULL	NULL	NULL	Ras-Rac pathway	GP		mediates					transcriptional activation	Process				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_3834	10066831	A domain containing the Cdc42/Rac interactive binding (CRIB) region of p65PAK inhibits transcriptional activation and cell transformation mediated by the Ras-Rac pathway.	bind
35277	3	10079	6	11	NULL	NULL	NULL	p65PAK	GP		inhibits			CRIB 		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_3834	10066831	A domain containing the Cdc42/Rac interactive binding (CRIB) region of p65PAK inhibits transcriptional activation and cell transformation mediated by the Ras-Rac pathway.	bind
35278	4	10079	6	11	NULL	NULL	NULL	CRIB	GP		is					Cdc42/Rac interactive binding 	GP				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_3834	10066831	A domain containing the Cdc42/Rac interactive binding (CRIB) region of p65PAK inhibits transcriptional activation and cell transformation mediated by the Ras-Rac pathway.	bind
35280	5	10079	6	11	NULL	NULL	NULL	p65PAK	GP		inhibits			CRIB		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_3834	10066831	A domain containing the Cdc42/Rac interactive binding (CRIB) region of p65PAK inhibits transcriptional activation and cell transformation mediated by the Ras-Rac pathway.	bind
42985	1	10079	7	11	NULL	NULL	NULL	p65PAK	GP		inhibits			CRIB region		statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_3834	10066831	A domain containing the Cdc42/Rac interactive binding (CRIB) region of p65PAK inhibits transcriptional activation and cell transformation mediated by the Ras-Rac pathway.	bind
42986	2	10079	7	11	NULL	NULL	NULL	Ras-Rac pathway	GP		mediates					cell transformation	Process				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_3834	10066831	A domain containing the Cdc42/Rac interactive binding (CRIB) region of p65PAK inhibits transcriptional activation and cell transformation mediated by the Ras-Rac pathway.	bind
42987	3	10079	7	11	NULL	NULL	NULL	p65PAK	GP		inhibits			CRIB region		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_3834	10066831	A domain containing the Cdc42/Rac interactive binding (CRIB) region of p65PAK inhibits transcriptional activation and cell transformation mediated by the Ras-Rac pathway.	bind
42988	4	10079	7	11	NULL	NULL	NULL	CRIB region 	GP		is					Cdc42/Rac interactive binding region	GP				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_3834	10066831	A domain containing the Cdc42/Rac interactive binding (CRIB) region of p65PAK inhibits transcriptional activation and cell transformation mediated by the Ras-Rac pathway.	bind
49526	5	10079	7	11	NULL	NULL	NULL	Ras-Rac pathway	GP		mediates					transcriptional activation	Process				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_3834	10066831	A domain containing the Cdc42/Rac interactive binding (CRIB) region of p65PAK inhibits transcriptional activation and cell transformation mediated by the Ras-Rac pathway.	bind
35281	1	10081	6	11	NULL	NULL	NULL	p21	GP		bind					PCNA	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_20865_s_18	16731526	A domain of p21 binds and inactivates PCNA ( ,  ).	bind
35282	2	10081	6	11	NULL	NULL	NULL	statement 1	Process		inactivates					PCNA	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_20865_s_18	16731526	A domain of p21 binds and inactivates PCNA ( ,  ).	bind
42989	1	10081	7	11	NULL	NULL	NULL	p21	GP		binds					PCNA	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_20865_s_18	16731526	A domain of p21 binds and inactivates PCNA ( ,  ).	bind
42990	2	10081	7	11	NULL	NULL	NULL	statement 1	Process		inactivates					PCNA	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_20865_s_18	16731526	A domain of p21 binds and inactivates PCNA ( ,  ).	bind
35615	1	10082	6	11	NULL	NULL	NULL	BTX	Chemical		bind					Na+ channel	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_56_2_404_s_35	10419561	A domain-interface allosteric model of BTX binding, similar to the domain-interface model of Ca2+-channel drug binding (interface of D3-S6 and D4-S6; Hockerman et al., 1997  ), was proposed for BTX binding to the Na+ channel, with its dimethylpyrrolidone carboxylic acid group directed toward D1-S6 and its steroid moiety toward D4-S6.	bind
35616	2	10082	6	11	NULL	NULL	NULL	BTX	Chemical		is directed towards			dimethylpyrrolidone carboxylic acid group					D1-S6		NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_56_2_404_s_35	10419561	A domain-interface allosteric model of BTX binding, similar to the domain-interface model of Ca2+-channel drug binding (interface of D3-S6 and D4-S6; Hockerman et al., 1997  ), was proposed for BTX binding to the Na+ channel, with its dimethylpyrrolidone carboxylic acid group directed toward D1-S6 and its steroid moiety toward D4-S6.	bind
36457	3	10082	6	11	NULL	NULL	NULL	BTX	Chemical		is directed towards			steroid moiety					D4-S6		NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_56_2_404_s_35	10419561	A domain-interface allosteric model of BTX binding, similar to the domain-interface model of Ca2+-channel drug binding (interface of D3-S6 and D4-S6; Hockerman et al., 1997  ), was proposed for BTX binding to the Na+ channel, with its dimethylpyrrolidone carboxylic acid group directed toward D1-S6 and its steroid moiety toward D4-S6.	bind
36458	4	10082	6	11	NULL	NULL	NULL	statement 2	Process		occurs simultaneously with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_56_2_404_s_35	10419561	A domain-interface allosteric model of BTX binding, similar to the domain-interface model of Ca2+-channel drug binding (interface of D3-S6 and D4-S6; Hockerman et al., 1997  ), was proposed for BTX binding to the Na+ channel, with its dimethylpyrrolidone carboxylic acid group directed toward D1-S6 and its steroid moiety toward D4-S6.	bind
36459	5	10082	6	11	NULL	NULL	NULL	statement 3	Process		occurs simultaneously with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_56_2_404_s_35	10419561	A domain-interface allosteric model of BTX binding, similar to the domain-interface model of Ca2+-channel drug binding (interface of D3-S6 and D4-S6; Hockerman et al., 1997  ), was proposed for BTX binding to the Na+ channel, with its dimethylpyrrolidone carboxylic acid group directed toward D1-S6 and its steroid moiety toward D4-S6.	bind
42991	1	10082	7	11	NULL	NULL	NULL	BTX	Chemical		bind					Na+ channel	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_56_2_404_s_35	10419561	A domain-interface allosteric model of BTX binding, similar to the domain-interface model of Ca2+-channel drug binding (interface of D3-S6 and D4-S6; Hockerman et al., 1997  ), was proposed for BTX binding to the Na+ channel, with its dimethylpyrrolidone carboxylic acid group directed toward D1-S6 and its steroid moiety toward D4-S6.	bind
42992	2	10082	7	11	NULL	NULL	NULL	BTX	Chemical		directed towards			dimethylpyrrolidone carboxylic acid group 					D1-S6 		NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_56_2_404_s_35	10419561	A domain-interface allosteric model of BTX binding, similar to the domain-interface model of Ca2+-channel drug binding (interface of D3-S6 and D4-S6; Hockerman et al., 1997  ), was proposed for BTX binding to the Na+ channel, with its dimethylpyrrolidone carboxylic acid group directed toward D1-S6 and its steroid moiety toward D4-S6.	bind
42993	3	10082	7	11	NULL	NULL	NULL	BTX	Chemical		directed towards			steroid moiety					D4-S6		NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_56_2_404_s_35	10419561	A domain-interface allosteric model of BTX binding, similar to the domain-interface model of Ca2+-channel drug binding (interface of D3-S6 and D4-S6; Hockerman et al., 1997  ), was proposed for BTX binding to the Na+ channel, with its dimethylpyrrolidone carboxylic acid group directed toward D1-S6 and its steroid moiety toward D4-S6.	bind
49527	4	10082	7	11	NULL	NULL	NULL	statement 2	Process		occurs simultaneously with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_56_2_404_s_35	10419561	A domain-interface allosteric model of BTX binding, similar to the domain-interface model of Ca2+-channel drug binding (interface of D3-S6 and D4-S6; Hockerman et al., 1997  ), was proposed for BTX binding to the Na+ channel, with its dimethylpyrrolidone carboxylic acid group directed toward D1-S6 and its steroid moiety toward D4-S6.	bind
49528	5	10082	7	11	NULL	NULL	NULL	statement 3	Process		occurs simultaneously with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_56_2_404_s_35	10419561	A domain-interface allosteric model of BTX binding, similar to the domain-interface model of Ca2+-channel drug binding (interface of D3-S6 and D4-S6; Hockerman et al., 1997  ), was proposed for BTX binding to the Na+ channel, with its dimethylpyrrolidone carboxylic acid group directed toward D1-S6 and its steroid moiety toward D4-S6.	bind
35344	1	10085	6	11	NULL	NULL	NULL	Ikaros gene	GP	dominant mutant	leads to					leukemia	MedicalFinding	development of			NULL		NULL	NULL	NULL	NULL	gw60_immunity_19_1_131_s_505	12871645	A dominant mutation in the Ikaros gene leads to rapid development of leukemia and lymphoma.	bind
35345	2	10085	6	11	NULL	NULL	NULL	Ikaros gene	GP	dominant mutant	leads to					lymphoma	MedicalFinding	development of			NULL		NULL	NULL	NULL	NULL	gw60_immunity_19_1_131_s_505	12871645	A dominant mutation in the Ikaros gene leads to rapid development of leukemia and lymphoma.	bind
43004	1	10085	7	11	NULL	NULL	NULL	Ikaros gene	GP	dominant mutant	leads to					leukemia	MedicalFinding	rapid development of			NULL		NULL	NULL	NULL	NULL	gw60_immunity_19_1_131_s_505	12871645	A dominant mutation in the Ikaros gene leads to rapid development of leukemia and lymphoma.	bind
43005	2	10085	7	11	NULL	NULL	NULL	Ikaros gene	GP	dominant mutant	leads to					lymphoma	MedicalFinding	rapid development of			NULL		NULL	NULL	NULL	NULL	gw60_immunity_19_1_131_s_505	12871645	A dominant mutation in the Ikaros gene leads to rapid development of leukemia and lymphoma.	bind
35346	1	10086	6	11	NULL	NULL	NULL	CK1epsilon	GP		bind					dsh	GP		PDZ domain		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_983_s_183	11524435	A dominant negative dsh mutant (Xdd1) that lacks the putative CK1epsilon binding domain (PDZ domain) fails to block the ability of CK1epsilon to stimulate wnt signaling in vivo ( Sokol, 1996), a result inconsistent with a model in which CK1epsilon mediates wnt signaling by binding to the PDZ domain of dsh.	bind
35347	2	10086	6	11	NULL	NULL	NULL	CK1epsilon	GP		mediates					wnt signaling	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_983_s_183	11524435	A dominant negative dsh mutant (Xdd1) that lacks the putative CK1epsilon binding domain (PDZ domain) fails to block the ability of CK1epsilon to stimulate wnt signaling in vivo ( Sokol, 1996), a result inconsistent with a model in which CK1epsilon mediates wnt signaling by binding to the PDZ domain of dsh.	bind
35348	3	10086	6	11	NULL	NULL	NULL	statement 1	Process		occurs via					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_983_s_183	11524435	A dominant negative dsh mutant (Xdd1) that lacks the putative CK1epsilon binding domain (PDZ domain) fails to block the ability of CK1epsilon to stimulate wnt signaling in vivo ( Sokol, 1996), a result inconsistent with a model in which CK1epsilon mediates wnt signaling by binding to the PDZ domain of dsh.	bind
35617	4	10086	6	11	NULL	NULL	NULL	Xdd1	GP		is a type of					dominant negative dsh mutant	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_983_s_183	11524435	A dominant negative dsh mutant (Xdd1) that lacks the putative CK1epsilon binding domain (PDZ domain) fails to block the ability of CK1epsilon to stimulate wnt signaling in vivo ( Sokol, 1996), a result inconsistent with a model in which CK1epsilon mediates wnt signaling by binding to the PDZ domain of dsh.	bind
35618	5	10086	6	11	NULL	NULL	NULL	Xdd1	GP		lacks							putative	PDZ domain		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_983_s_183	11524435	A dominant negative dsh mutant (Xdd1) that lacks the putative CK1epsilon binding domain (PDZ domain) fails to block the ability of CK1epsilon to stimulate wnt signaling in vivo ( Sokol, 1996), a result inconsistent with a model in which CK1epsilon mediates wnt signaling by binding to the PDZ domain of dsh.	bind
35619	6	10086	6	11	NULL	NULL	NULL	CK1epsilon binding domain	GP		is					PDZ domain	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_983_s_183	11524435	A dominant negative dsh mutant (Xdd1) that lacks the putative CK1epsilon binding domain (PDZ domain) fails to block the ability of CK1epsilon to stimulate wnt signaling in vivo ( Sokol, 1996), a result inconsistent with a model in which CK1epsilon mediates wnt signaling by binding to the PDZ domain of dsh.	bind
35620	7	10086	6	11	NULL	NULL	NULL	statement 5	Process		fails to block					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_983_s_183	11524435	A dominant negative dsh mutant (Xdd1) that lacks the putative CK1epsilon binding domain (PDZ domain) fails to block the ability of CK1epsilon to stimulate wnt signaling in vivo ( Sokol, 1996), a result inconsistent with a model in which CK1epsilon mediates wnt signaling by binding to the PDZ domain of dsh.	bind
49529	8	10086	6	11	NULL	NULL	NULL	CK1epsilon	GP		stimulates					wnt signaling	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_983_s_183	11524435	A dominant negative dsh mutant (Xdd1) that lacks the putative CK1epsilon binding domain (PDZ domain) fails to block the ability of CK1epsilon to stimulate wnt signaling in vivo ( Sokol, 1996), a result inconsistent with a model in which CK1epsilon mediates wnt signaling by binding to the PDZ domain of dsh.	bind
43007	1	10086	7	11	NULL	NULL	NULL	CK1epsilon	GP		stimulate					wnt signaling	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_983_s_183	11524435	A dominant negative dsh mutant (Xdd1) that lacks the putative CK1epsilon binding domain (PDZ domain) fails to block the ability of CK1epsilon to stimulate wnt signaling in vivo ( Sokol, 1996), a result inconsistent with a model in which CK1epsilon mediates wnt signaling by binding to the PDZ domain of dsh.	bind
43008	2	10086	7	11	NULL	NULL	NULL	CK1epsilon 	GP		mediates					wnt signaling	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_983_s_183	11524435	A dominant negative dsh mutant (Xdd1) that lacks the putative CK1epsilon binding domain (PDZ domain) fails to block the ability of CK1epsilon to stimulate wnt signaling in vivo ( Sokol, 1996), a result inconsistent with a model in which CK1epsilon mediates wnt signaling by binding to the PDZ domain of dsh.	bind
43024	3	10086	7	11	NULL	NULL	NULL	Xdd1	GP		lacks							putative	 PDZ domain		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_983_s_183	11524435	A dominant negative dsh mutant (Xdd1) that lacks the putative CK1epsilon binding domain (PDZ domain) fails to block the ability of CK1epsilon to stimulate wnt signaling in vivo ( Sokol, 1996), a result inconsistent with a model in which CK1epsilon mediates wnt signaling by binding to the PDZ domain of dsh.	bind
43027	4	10086	7	11	NULL	NULL	NULL	statement 3	Process		fails to block					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_983_s_183	11524435	A dominant negative dsh mutant (Xdd1) that lacks the putative CK1epsilon binding domain (PDZ domain) fails to block the ability of CK1epsilon to stimulate wnt signaling in vivo ( Sokol, 1996), a result inconsistent with a model in which CK1epsilon mediates wnt signaling by binding to the PDZ domain of dsh.	bind
43028	5	10086	7	11	NULL	NULL	NULL	CK1epsilon	GP		bind					dsh	GP		PDZ domain		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_983_s_183	11524435	A dominant negative dsh mutant (Xdd1) that lacks the putative CK1epsilon binding domain (PDZ domain) fails to block the ability of CK1epsilon to stimulate wnt signaling in vivo ( Sokol, 1996), a result inconsistent with a model in which CK1epsilon mediates wnt signaling by binding to the PDZ domain of dsh.	bind
43029	6	10086	7	11	NULL	NULL	NULL	statement 2	Process		occurs via					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_983_s_183	11524435	A dominant negative dsh mutant (Xdd1) that lacks the putative CK1epsilon binding domain (PDZ domain) fails to block the ability of CK1epsilon to stimulate wnt signaling in vivo ( Sokol, 1996), a result inconsistent with a model in which CK1epsilon mediates wnt signaling by binding to the PDZ domain of dsh.	bind
43030	7	10086	7	11	NULL	NULL	NULL	Xdd1	GP		is a type of					dominant negative dsh mutant	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_983_s_183	11524435	A dominant negative dsh mutant (Xdd1) that lacks the putative CK1epsilon binding domain (PDZ domain) fails to block the ability of CK1epsilon to stimulate wnt signaling in vivo ( Sokol, 1996), a result inconsistent with a model in which CK1epsilon mediates wnt signaling by binding to the PDZ domain of dsh.	bind
49530	8	10086	7	11	NULL	NULL	NULL	CK1epsilon binding domain	GP		is					PDZ domain	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_983_s_183	11524435	A dominant negative dsh mutant (Xdd1) that lacks the putative CK1epsilon binding domain (PDZ domain) fails to block the ability of CK1epsilon to stimulate wnt signaling in vivo ( Sokol, 1996), a result inconsistent with a model in which CK1epsilon mediates wnt signaling by binding to the PDZ domain of dsh.	bind
35349	1	10087	6	11	NULL	NULL	NULL	peroxisome proliferator-activated receptor-gamma	GP	dominant negative;; knock-in mouse	exhibits					metabolic syndrome	MedicalFinding	features of 			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_17_17118_s_1	15716267	A dominant negative peroxisome proliferator-activated receptor-gamma knock-in mouse exhibits features of the metabolic syndrome.	bind
43031	1	10087	7	11	NULL	NULL	NULL	peroxisome proliferator-activated receptor-gamma 	GP	dominant negative;;knock-in mouse	exhibits					metabolic syndrome	MedicalFinding	features of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_17_17118_s_1	15716267	A dominant negative peroxisome proliferator-activated receptor-gamma knock-in mouse exhibits features of the metabolic syndrome.	bind
35621	1	10088	6	11	NULL	NULL	NULL	CD27	GP		induces					NF-kappaB	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_13353_s_111	9582383	A Dominant Negative TRAF2 or TRAF5 Block NF-kappa B Activation Induced by CD27-- To determine whether TRAF2 and TRAF5 are involved in NF-kappaB activation by CD27, we tested whether N-terminal truncated mutants of TRAF2 and TRAF5 would act as dominant negative mutants based on previous results that showed that the zinc binding domain of TRAF2 and TRAF5 is required for NF-kappaB activation ( 9,  12).	bind
35622	2	10088	6	11	NULL	NULL	NULL	TRAF2	GP		is required for			zinc binding domain		NF-kappaB	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_13353_s_111	9582383	A Dominant Negative TRAF2 or TRAF5 Block NF-kappa B Activation Induced by CD27-- To determine whether TRAF2 and TRAF5 are involved in NF-kappaB activation by CD27, we tested whether N-terminal truncated mutants of TRAF2 and TRAF5 would act as dominant negative mutants based on previous results that showed that the zinc binding domain of TRAF2 and TRAF5 is required for NF-kappaB activation ( 9,  12).	bind
35623	3	10088	6	11	NULL	NULL	NULL	TRAF5	GP		is required for			zinc binding domain		NF-kappaB	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_13353_s_111	9582383	A Dominant Negative TRAF2 or TRAF5 Block NF-kappa B Activation Induced by CD27-- To determine whether TRAF2 and TRAF5 are involved in NF-kappaB activation by CD27, we tested whether N-terminal truncated mutants of TRAF2 and TRAF5 would act as dominant negative mutants based on previous results that showed that the zinc binding domain of TRAF2 and TRAF5 is required for NF-kappaB activation ( 9,  12).	bind
35624	4	10088	6	11	NULL	NULL	NULL	TRAF2	GP	dominant-negative	blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_13353_s_111	9582383	A Dominant Negative TRAF2 or TRAF5 Block NF-kappa B Activation Induced by CD27-- To determine whether TRAF2 and TRAF5 are involved in NF-kappaB activation by CD27, we tested whether N-terminal truncated mutants of TRAF2 and TRAF5 would act as dominant negative mutants based on previous results that showed that the zinc binding domain of TRAF2 and TRAF5 is required for NF-kappaB activation ( 9,  12).	bind
35625	5	10088	6	11	NULL	NULL	NULL	TRAF5	GP	dominant-negative	blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_13353_s_111	9582383	A Dominant Negative TRAF2 or TRAF5 Block NF-kappa B Activation Induced by CD27-- To determine whether TRAF2 and TRAF5 are involved in NF-kappaB activation by CD27, we tested whether N-terminal truncated mutants of TRAF2 and TRAF5 would act as dominant negative mutants based on previous results that showed that the zinc binding domain of TRAF2 and TRAF5 is required for NF-kappaB activation ( 9,  12).	bind
43033	1	10088	7	11	NULL	NULL	NULL	TRAF2	GP		is required for			zinc binding domain 		NF-kappaB	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_13353_s_111	9582383	A Dominant Negative TRAF2 or TRAF5 Block NF-kappa B Activation Induced by CD27-- To determine whether TRAF2 and TRAF5 are involved in NF-kappaB activation by CD27, we tested whether N-terminal truncated mutants of TRAF2 and TRAF5 would act as dominant negative mutants based on previous results that showed that the zinc binding domain of TRAF2 and TRAF5 is required for NF-kappaB activation ( 9,  12).	bind
43034	2	10088	7	11	NULL	NULL	NULL	TRAF5	GP		is required for			zinc binding domain 		NF-kappaB	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_13353_s_111	9582383	A Dominant Negative TRAF2 or TRAF5 Block NF-kappa B Activation Induced by CD27-- To determine whether TRAF2 and TRAF5 are involved in NF-kappaB activation by CD27, we tested whether N-terminal truncated mutants of TRAF2 and TRAF5 would act as dominant negative mutants based on previous results that showed that the zinc binding domain of TRAF2 and TRAF5 is required for NF-kappaB activation ( 9,  12).	bind
43035	3	10088	7	11	NULL	NULL	NULL	CD27	GP		induce					NF-kappaB	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_13353_s_111	9582383	A Dominant Negative TRAF2 or TRAF5 Block NF-kappa B Activation Induced by CD27-- To determine whether TRAF2 and TRAF5 are involved in NF-kappaB activation by CD27, we tested whether N-terminal truncated mutants of TRAF2 and TRAF5 would act as dominant negative mutants based on previous results that showed that the zinc binding domain of TRAF2 and TRAF5 is required for NF-kappaB activation ( 9,  12).	bind
43036	4	10088	7	11	NULL	NULL	NULL	TRAF2	GP	dominant-negative	blocks					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_13353_s_111	9582383	A Dominant Negative TRAF2 or TRAF5 Block NF-kappa B Activation Induced by CD27-- To determine whether TRAF2 and TRAF5 are involved in NF-kappaB activation by CD27, we tested whether N-terminal truncated mutants of TRAF2 and TRAF5 would act as dominant negative mutants based on previous results that showed that the zinc binding domain of TRAF2 and TRAF5 is required for NF-kappaB activation ( 9,  12).	bind
43037	5	10088	7	11	NULL	NULL	NULL	TRAF5	GP	dominant-negative	blocks					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_13353_s_111	9582383	A Dominant Negative TRAF2 or TRAF5 Block NF-kappa B Activation Induced by CD27-- To determine whether TRAF2 and TRAF5 are involved in NF-kappaB activation by CD27, we tested whether N-terminal truncated mutants of TRAF2 and TRAF5 would act as dominant negative mutants based on previous results that showed that the zinc binding domain of TRAF2 and TRAF5 is required for NF-kappaB activation ( 9,  12).	bind
35350	1	10089	6	11	NULL	NULL	NULL	FADD-DN	GP		lacks								death effector domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_41_25783_s_84	9325306	A dominant negative version of FADD (FADD-DN) that lacks the death effector domain and is therefore unable to recruit FLICE inhibits cell death induced by all three receptors (CD95, TNFR1, and DR3).	bind
35351	2	10089	6	11	NULL	NULL	NULL	FADD-DN	GP		is unable to recruit					FLICE	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_41_25783_s_84	9325306	A dominant negative version of FADD (FADD-DN) that lacks the death effector domain and is therefore unable to recruit FLICE inhibits cell death induced by all three receptors (CD95, TNFR1, and DR3).	bind
36460	3	10089	6	11	NULL	NULL	NULL	FADD-DN	GP		inhibits					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_41_25783_s_84	9325306	A dominant negative version of FADD (FADD-DN) that lacks the death effector domain and is therefore unable to recruit FLICE inhibits cell death induced by all three receptors (CD95, TNFR1, and DR3).	bind
36461	4	10089	6	11	NULL	NULL	NULL	cell death	Process		is induced by					CD95	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_41_25783_s_84	9325306	A dominant negative version of FADD (FADD-DN) that lacks the death effector domain and is therefore unable to recruit FLICE inhibits cell death induced by all three receptors (CD95, TNFR1, and DR3).	bind
36462	5	10089	6	11	NULL	NULL	NULL	cell death	Process		is induced by					TNFR1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_41_25783_s_84	9325306	A dominant negative version of FADD (FADD-DN) that lacks the death effector domain and is therefore unable to recruit FLICE inhibits cell death induced by all three receptors (CD95, TNFR1, and DR3).	bind
36463	6	10089	6	11	NULL	NULL	NULL	cell death 	Process		is induced by					DR3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_41_25783_s_84	9325306	A dominant negative version of FADD (FADD-DN) that lacks the death effector domain and is therefore unable to recruit FLICE inhibits cell death induced by all three receptors (CD95, TNFR1, and DR3).	bind
49536	7	10089	6	11	NULL	NULL	NULL	FADD-DN	GP		inhibits					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_41_25783_s_84	9325306	A dominant negative version of FADD (FADD-DN) that lacks the death effector domain and is therefore unable to recruit FLICE inhibits cell death induced by all three receptors (CD95, TNFR1, and DR3).	bind
49537	8	10089	6	11	NULL	NULL	NULL	FADD-DN	GP		inhibits					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_41_25783_s_84	9325306	A dominant negative version of FADD (FADD-DN) that lacks the death effector domain and is therefore unable to recruit FLICE inhibits cell death induced by all three receptors (CD95, TNFR1, and DR3).	bind
57319	9	10089	6	11	NULL	NULL	NULL	FADD-DN	GP		is					dominant negative mutant of FADD	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_41_25783_s_84	9325306	A dominant negative version of FADD (FADD-DN) that lacks the death effector domain and is therefore unable to recruit FLICE inhibits cell death induced by all three receptors (CD95, TNFR1, and DR3).	bind
43038	1	10089	7	11	NULL	NULL	NULL	FADD-DN	GP		lacks								death effector domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_41_25783_s_84	9325306	A dominant negative version of FADD (FADD-DN) that lacks the death effector domain and is therefore unable to recruit FLICE inhibits cell death induced by all three receptors (CD95, TNFR1, and DR3).	bind
43039	2	10089	7	11	NULL	NULL	NULL	statement 1	Process		is unable to recruit					FLICE	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_41_25783_s_84	9325306	A dominant negative version of FADD (FADD-DN) that lacks the death effector domain and is therefore unable to recruit FLICE inhibits cell death induced by all three receptors (CD95, TNFR1, and DR3).	bind
43040	3	10089	7	11	NULL	NULL	NULL	cell death	Process		induced by					CD95	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_41_25783_s_84	9325306	A dominant negative version of FADD (FADD-DN) that lacks the death effector domain and is therefore unable to recruit FLICE inhibits cell death induced by all three receptors (CD95, TNFR1, and DR3).	bind
43061	4	10089	7	11	NULL	NULL	NULL	cell death	Process		induced by					TNFR1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_41_25783_s_84	9325306	A dominant negative version of FADD (FADD-DN) that lacks the death effector domain and is therefore unable to recruit FLICE inhibits cell death induced by all three receptors (CD95, TNFR1, and DR3).	bind
43062	5	10089	7	11	NULL	NULL	NULL	cell death	Process		induced by					DR3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_41_25783_s_84	9325306	A dominant negative version of FADD (FADD-DN) that lacks the death effector domain and is therefore unable to recruit FLICE inhibits cell death induced by all three receptors (CD95, TNFR1, and DR3).	bind
43063	6	10089	7	11	NULL	NULL	NULL	FADD-DN	GP		inhibits					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_41_25783_s_84	9325306	A dominant negative version of FADD (FADD-DN) that lacks the death effector domain and is therefore unable to recruit FLICE inhibits cell death induced by all three receptors (CD95, TNFR1, and DR3).	bind
43064	7	10089	7	11	NULL	NULL	NULL	FADD-DN	GP		inhibits					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_41_25783_s_84	9325306	A dominant negative version of FADD (FADD-DN) that lacks the death effector domain and is therefore unable to recruit FLICE inhibits cell death induced by all three receptors (CD95, TNFR1, and DR3).	bind
43065	8	10089	7	11	NULL	NULL	NULL	FADD-DN	GP		inhibits					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_41_25783_s_84	9325306	A dominant negative version of FADD (FADD-DN) that lacks the death effector domain and is therefore unable to recruit FLICE inhibits cell death induced by all three receptors (CD95, TNFR1, and DR3).	bind
43066	9	10089	7	11	NULL	NULL	NULL	FADD-DN	GP		is					dominant negative mutant of FADD	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_41_25783_s_84	9325306	A dominant negative version of FADD (FADD-DN) that lacks the death effector domain and is therefore unable to recruit FLICE inhibits cell death induced by all three receptors (CD95, TNFR1, and DR3).	bind
35352	1	10090	6	11	NULL	NULL	NULL	N17Cdc42	GP		does not bind					WASP	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_1_70_s_45	8805223	A dominant-negative form of Cdc42 (N17Cdc42) also failed to bind WASP, suggesting that WASP specifically recognized the GTP-bound conformation of Cdc42.	bind
35353	2	10090	6	11	NULL	NULL	NULL	dominant-negative form of Cdc42	GP		is					N17Cdc42	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_1_70_s_45	8805223	A dominant-negative form of Cdc42 (N17Cdc42) also failed to bind WASP, suggesting that WASP specifically recognized the GTP-bound conformation of Cdc42.	bind
35354	3	10090	6	11	NULL	NULL	NULL	Cdc42	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_1_70_s_45	8805223	A dominant-negative form of Cdc42 (N17Cdc42) also failed to bind WASP, suggesting that WASP specifically recognized the GTP-bound conformation of Cdc42.	bind
35355	4	10090	6	11	NULL	NULL	NULL	WASP	GP		recognizes		specifically			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_1_70_s_45	8805223	A dominant-negative form of Cdc42 (N17Cdc42) also failed to bind WASP, suggesting that WASP specifically recognized the GTP-bound conformation of Cdc42.	bind
43067	1	10090	7	11	NULL	NULL	NULL	N17Cdc42	GP		fails to bind					WASP	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_1_70_s_45	8805223	A dominant-negative form of Cdc42 (N17Cdc42) also failed to bind WASP, suggesting that WASP specifically recognized the GTP-bound conformation of Cdc42.	bind
43068	2	10090	7	11	NULL	NULL	NULL	Cdc42	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_1_70_s_45	8805223	A dominant-negative form of Cdc42 (N17Cdc42) also failed to bind WASP, suggesting that WASP specifically recognized the GTP-bound conformation of Cdc42.	bind
43069	3	10090	7	11	NULL	NULL	NULL	WASP	GP		recognize		specifically			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_1_70_s_45	8805223	A dominant-negative form of Cdc42 (N17Cdc42) also failed to bind WASP, suggesting that WASP specifically recognized the GTP-bound conformation of Cdc42.	bind
43070	4	10090	7	11	NULL	NULL	NULL	dominant-negative form of Cdc42	GP		is					N17Cdc42	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_1_70_s_45	8805223	A dominant-negative form of Cdc42 (N17Cdc42) also failed to bind WASP, suggesting that WASP specifically recognized the GTP-bound conformation of Cdc42.	bind
35356	1	10091	6	11	NULL	NULL	NULL	Ras	GP	dominant-negative mutant	bind		tightly	S17N		Ras-GEF	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_46_27880_s_188	7499262	A dominant-negative mutant  Ras(S17N), which binds to Ras-GEFs tightly to prevent its action toward  endogenous Ras, has been utilized widely to evaluate whether Ras is  essential for a particular signal transduction pathway (Feig and  Cooper, 1988).	bind
43078	1	10091	7	11	NULL	NULL	NULL	Ras	GP	\tdominant-negative mutant	binds to		tightly	S17N		Ras-GEFs	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_46_27880_s_188	7499262	A dominant-negative mutant  Ras(S17N), which binds to Ras-GEFs tightly to prevent its action toward  endogenous Ras, has been utilized widely to evaluate whether Ras is  essential for a particular signal transduction pathway (Feig and  Cooper, 1988).	bind
35357	1	10092	6	11	NULL	NULL	NULL	cyclin D1	GP	dominant-negative mutant	bind			T156A		Cdk4	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_2251_s_309	10022912	A dominant-negative mutant of cyclin D1 (T156A) can still bind to cdk4, but the complex is not imported into the nucleus ( 14), suggesting that a conformational state is recognized by such a carrier protein.	bind
49552	2	10092	6	11	NULL	NULL	NULL	statement 1	Process		is not imported into					nucleus	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_2251_s_309	10022912	A dominant-negative mutant of cyclin D1 (T156A) can still bind to cdk4, but the complex is not imported into the nucleus ( 14), suggesting that a conformational state is recognized by such a carrier protein.	bind
43084	1	10092	7	11	NULL	NULL	NULL	cyclin D1	GP	dominant-negative mutant 	bind			T156A		cdk4	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_2251_s_309	10022912	A dominant-negative mutant of cyclin D1 (T156A) can still bind to cdk4, but the complex is not imported into the nucleus ( 14), suggesting that a conformational state is recognized by such a carrier protein.	bind
43085	2	10092	7	11	NULL	NULL	NULL	statement 1	Process		is not imported into					nucleus	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_2251_s_309	10022912	A dominant-negative mutant of cyclin D1 (T156A) can still bind to cdk4, but the complex is not imported into the nucleus ( 14), suggesting that a conformational state is recognized by such a carrier protein.	bind
35358	1	10094	6	11	NULL	NULL	NULL	Rab11	GP	\tdominant-negative mutant	bind		constitutively	S25N		GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_16_6065_s_365	16880518	A dominant-negative Rab11 mutant, Rab11 (S25N), which constitutively binds GDP, and blocks endosomal trafficking ( ) was coexpressed with GFP-GLUT4 and HA-72-5ptase (Fig.  8C).	bind
35359	2	10094	6	11	NULL	NULL	NULL	statement 1	Process		blocks					endosomal trafficking	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_16_6065_s_365	16880518	A dominant-negative Rab11 mutant, Rab11 (S25N), which constitutively binds GDP, and blocks endosomal trafficking ( ) was coexpressed with GFP-GLUT4 and HA-72-5ptase (Fig.  8C).	bind
43088	1	10094	7	11	NULL	NULL	NULL	Rab11	GP	\tdominant-negative mutant	binds		constitutively	S25N		GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_16_6065_s_365	16880518	A dominant-negative Rab11 mutant, Rab11 (S25N), which constitutively binds GDP, and blocks endosomal trafficking ( ) was coexpressed with GFP-GLUT4 and HA-72-5ptase (Fig.  8C).	bind
43089	2	10094	7	11	NULL	NULL	NULL	statement 1	Process		blocks					endosomal trafficking	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_16_6065_s_365	16880518	A dominant-negative Rab11 mutant, Rab11 (S25N), which constitutively binds GDP, and blocks endosomal trafficking ( ) was coexpressed with GFP-GLUT4 and HA-72-5ptase (Fig.  8C).	bind
35626	1	10095	6	11	NULL	NULL	NULL	TRAF2	GP		bind					CD40	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_4_379_s_173	9133417	A dominant-negative TRAF3, which has the potential to displace the binding of both TRAF3 and TRAF2 to CD40 (  Cheng et al. 1995  ; Rothe et al. 1995  ), was previously shown to inhibit CD40-mediated expression of CD23 but not of ICAM-1 ( Cheng et al. 1995  ).	bind
35627	2	10095	6	11	NULL	NULL	NULL	TRAF3	GP		bind					CD40	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_4_379_s_173	9133417	A dominant-negative TRAF3, which has the potential to displace the binding of both TRAF3 and TRAF2 to CD40 (  Cheng et al. 1995  ; Rothe et al. 1995  ), was previously shown to inhibit CD40-mediated expression of CD23 but not of ICAM-1 ( Cheng et al. 1995  ).	bind
35628	3	10095	6	11	NULL	NULL	NULL	TRAF3	GP	dominant-negative	displaces					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_4_379_s_173	9133417	A dominant-negative TRAF3, which has the potential to displace the binding of both TRAF3 and TRAF2 to CD40 (  Cheng et al. 1995  ; Rothe et al. 1995  ), was previously shown to inhibit CD40-mediated expression of CD23 but not of ICAM-1 ( Cheng et al. 1995  ).	bind
35629	4	10095	6	11	NULL	NULL	NULL	TRAF3	GP	dominant-negative	displaces					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_4_379_s_173	9133417	A dominant-negative TRAF3, which has the potential to displace the binding of both TRAF3 and TRAF2 to CD40 (  Cheng et al. 1995  ; Rothe et al. 1995  ), was previously shown to inhibit CD40-mediated expression of CD23 but not of ICAM-1 ( Cheng et al. 1995  ).	bind
35630	5	10095	6	11	NULL	NULL	NULL	CD23	GP	expression of	is mediated by					CD40	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_4_379_s_173	9133417	A dominant-negative TRAF3, which has the potential to displace the binding of both TRAF3 and TRAF2 to CD40 (  Cheng et al. 1995  ; Rothe et al. 1995  ), was previously shown to inhibit CD40-mediated expression of CD23 but not of ICAM-1 ( Cheng et al. 1995  ).	bind
35631	6	10095	6	11	NULL	NULL	NULL	TRAF3	GP	dominant-negative	inhibits					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_4_379_s_173	9133417	A dominant-negative TRAF3, which has the potential to displace the binding of both TRAF3 and TRAF2 to CD40 (  Cheng et al. 1995  ; Rothe et al. 1995  ), was previously shown to inhibit CD40-mediated expression of CD23 but not of ICAM-1 ( Cheng et al. 1995  ).	bind
35632	7	10095	6	11	NULL	NULL	NULL	TRAF3	GP	dominant-negative	does not inhibit					ICAM-1	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_4_379_s_173	9133417	A dominant-negative TRAF3, which has the potential to displace the binding of both TRAF3 and TRAF2 to CD40 (  Cheng et al. 1995  ; Rothe et al. 1995  ), was previously shown to inhibit CD40-mediated expression of CD23 but not of ICAM-1 ( Cheng et al. 1995  ).	bind
43091	1	10095	7	11	NULL	NULL	NULL	TRAF3 	GP		bind					CD40	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_4_379_s_173	9133417	A dominant-negative TRAF3, which has the potential to displace the binding of both TRAF3 and TRAF2 to CD40 (  Cheng et al. 1995  ; Rothe et al. 1995  ), was previously shown to inhibit CD40-mediated expression of CD23 but not of ICAM-1 ( Cheng et al. 1995  ).	bind
43092	2	10095	7	11	NULL	NULL	NULL	TRAF2	GP		bind					CD40	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_4_379_s_173	9133417	A dominant-negative TRAF3, which has the potential to displace the binding of both TRAF3 and TRAF2 to CD40 (  Cheng et al. 1995  ; Rothe et al. 1995  ), was previously shown to inhibit CD40-mediated expression of CD23 but not of ICAM-1 ( Cheng et al. 1995  ).	bind
43093	3	10095	7	11	NULL	NULL	NULL	TRAF3	GP	dominant-negative	displace					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_4_379_s_173	9133417	A dominant-negative TRAF3, which has the potential to displace the binding of both TRAF3 and TRAF2 to CD40 (  Cheng et al. 1995  ; Rothe et al. 1995  ), was previously shown to inhibit CD40-mediated expression of CD23 but not of ICAM-1 ( Cheng et al. 1995  ).	bind
43094	4	10095	7	11	NULL	NULL	NULL	TRAF3	GP	dominant-negative	displace					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_4_379_s_173	9133417	A dominant-negative TRAF3, which has the potential to displace the binding of both TRAF3 and TRAF2 to CD40 (  Cheng et al. 1995  ; Rothe et al. 1995  ), was previously shown to inhibit CD40-mediated expression of CD23 but not of ICAM-1 ( Cheng et al. 1995  ).	bind
43095	5	10095	7	11	NULL	NULL	NULL	CD23	GP	expression of	is mediated by					CD40	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_4_379_s_173	9133417	A dominant-negative TRAF3, which has the potential to displace the binding of both TRAF3 and TRAF2 to CD40 (  Cheng et al. 1995  ; Rothe et al. 1995  ), was previously shown to inhibit CD40-mediated expression of CD23 but not of ICAM-1 ( Cheng et al. 1995  ).	bind
43097	6	10095	7	11	NULL	NULL	NULL	TRAF3	GP	dominant-negative	inhibits					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_4_379_s_173	9133417	A dominant-negative TRAF3, which has the potential to displace the binding of both TRAF3 and TRAF2 to CD40 (  Cheng et al. 1995  ; Rothe et al. 1995  ), was previously shown to inhibit CD40-mediated expression of CD23 but not of ICAM-1 ( Cheng et al. 1995  ).	bind
43099	7	10095	7	11	NULL	NULL	NULL	TRAF3	GP	dominant-negative	does not inhibit					ICAM-1	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_4_379_s_173	9133417	A dominant-negative TRAF3, which has the potential to displace the binding of both TRAF3 and TRAF2 to CD40 (  Cheng et al. 1995  ; Rothe et al. 1995  ), was previously shown to inhibit CD40-mediated expression of CD23 but not of ICAM-1 ( Cheng et al. 1995  ).	bind
35360	1	10096	6	11	NULL	NULL	NULL	CD80Fc	GP		bind					CD152-Fc	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_10149_s_144	15598660	A dose response exhibiting greater decrease in the percentage of binding of CD80Fc to CD152-Fc was observed with increasing concentrations of CD80-CAP1 ( Fig. 4 B).	bind
35361	2	10096	6	11	NULL	NULL	NULL	CD80-CAP1	GP	increasing concentrations of	decreases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_10149_s_144	15598660	A dose response exhibiting greater decrease in the percentage of binding of CD80Fc to CD152-Fc was observed with increasing concentrations of CD80-CAP1 ( Fig. 4 B).	bind
43101	1	10096	7	11	NULL	NULL	NULL	CD80Fc	GP		binds					CD152-Fc	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_10149_s_144	15598660	A dose response exhibiting greater decrease in the percentage of binding of CD80Fc to CD152-Fc was observed with increasing concentrations of CD80-CAP1 ( Fig. 4 B).	bind
49553	2	10096	7	11	NULL	NULL	NULL	CD80-CAP1	GP	increasing concentrations of	decreases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_10149_s_144	15598660	A dose response exhibiting greater decrease in the percentage of binding of CD80Fc to CD152-Fc was observed with increasing concentrations of CD80-CAP1 ( Fig. 4 B).	bind
35362	1	10097	6	11	NULL	NULL	NULL	tra-1	GP		interacts with		dose-sensitively			ehn-3	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_131_17_4333_s_229	15294864	A dose sensitive interaction between  tra-1 and  ehn-3   In constructing  tra-1(e1099); ehn-3(q689), we found that  tra-1 is a dominant enhancer of the  ehn-3 gonadogenesis defects.	bind
35364	3	10097	6	11	NULL	NULL	NULL	tra-1	GP		is an enhancer of		dominant			ehn-3	GP	gonadogenesis defects of			NULL		NULL	NULL	NULL	NULL	gw70_development_131_17_4333_s_229	15294864	A dose sensitive interaction between  tra-1 and  ehn-3   In constructing  tra-1(e1099); ehn-3(q689), we found that  tra-1 is a dominant enhancer of the  ehn-3 gonadogenesis defects.	bind
43102	1	10097	7	11	NULL	NULL	NULL	tra-1 	GP		interacts with		dose-sensitively			ehn-3	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_131_17_4333_s_229	15294864	A dose sensitive interaction between  tra-1 and  ehn-3   In constructing  tra-1(e1099); ehn-3(q689), we found that  tra-1 is a dominant enhancer of the  ehn-3 gonadogenesis defects.	bind
43103	2	10097	7	11	NULL	NULL	NULL	tra-1	GP		is an enhancer of		dominant			ehn-3	GP	gonadogenesis defects of			NULL		NULL	NULL	NULL	NULL	gw70_development_131_17_4333_s_229	15294864	A dose sensitive interaction between  tra-1 and  ehn-3   In constructing  tra-1(e1099); ehn-3(q689), we found that  tra-1 is a dominant enhancer of the  ehn-3 gonadogenesis defects.	bind
35365	1	10098	6	11	NULL	NULL	NULL	H-kininogen	GP	biotinylated	bind		dose dependently			EA.hy926 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_13040_s_154	8662673	A dose-dependent binding of biotinylated H-kininogen to EA.hy926 cells was observed at concentrations of  10 nM.	bind
43104	1	10098	7	11	NULL	NULL	NULL	H-kininogen	GP	biotinylated	bind		dose-dependently			EA.hy926 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_22_13040_s_154	8662673	A dose-dependent binding of biotinylated H-kininogen to EA.hy926 cells was observed at concentrations of  10 nM.	bind
35366	1	10100	6	11	NULL	NULL	NULL	nuclear factor	GP		bind		high affinity			Glut3	GP	mouse;; unlabeled		bp 149 to 124	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_42_27474_s_182	9765277	A dose-dependent displacement of the band shifts with the unlabeled bp  149 to  124 region of the mouse Glut 3 established a relatively high affinity binding of nuclear factor(s) to this region (Fig.  3 C).	bind
43105	1	10100	7	11	NULL	NULL	NULL	nuclear factors	GP		bind		high affinity			Glut 3 	GP	mouse;;unlabeled		bp 149 to 124	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_42_27474_s_182	9765277	A dose-dependent displacement of the band shifts with the unlabeled bp  149 to  124 region of the mouse Glut 3 established a relatively high affinity binding of nuclear factor(s) to this region (Fig.  3 C).	bind
35367	1	10101	6	11	NULL	NULL	NULL	HSP90	GP		bind		dose dependently			eNOS	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_11_9339_s_154	12519764	A dose-dependent increase in HSP90 binding to eNOS also was observed at high Ca2+ concentration.	bind
35368	2	10101	6	11	NULL	NULL	NULL	statement 1	Process		in the presence of					Ca2+ 	Chemical	high concentrations of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_11_9339_s_154	12519764	A dose-dependent increase in HSP90 binding to eNOS also was observed at high Ca2+ concentration.	bind
43107	1	10101	7	11	NULL	NULL	NULL	HSP90	GP		bind		dose-dependently			eNOS	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_11_9339_s_154	12519764	A dose-dependent increase in HSP90 binding to eNOS also was observed at high Ca2+ concentration.	bind
43108	2	10101	7	11	NULL	NULL	NULL	statement 1	Process		 in the presence of					Ca2+	Chemical	high concentrations of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_11_9339_s_154	12519764	A dose-dependent increase in HSP90 binding to eNOS also was observed at high Ca2+ concentration.	bind
35369	1	10102	6	11	NULL	NULL	NULL	anti - HSP-65	GP		bind					HSP-65	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_505_s_108	10073950	A dose-dependent inhibition of anti - HSP-65 binding to HSP-65 - coated plates was evident.	bind
43109	1	10102	7	11	NULL	NULL	NULL	anti - HSP-65	GP		bind					HSP-65	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_505_s_108	10073950	A dose-dependent inhibition of anti - HSP-65 binding to HSP-65 - coated plates was evident.	bind
35370	1	10103	6	11	NULL	NULL	NULL	CRP	GP		bind					E-LDL	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2348_s_143	10521363	A dose-dependent inhibition of CRP binding to E-LDL was observed, indicating that CRP interacted with its classical ligand 25 26  within the degraded LDL particles.	bind
35371	2	10103	6	11	NULL	NULL	NULL	CRP	GP		interacts with					classical ligand	Chemical				NULL	degraded LDL particle	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2348_s_143	10521363	A dose-dependent inhibition of CRP binding to E-LDL was observed, indicating that CRP interacted with its classical ligand 25 26  within the degraded LDL particles.	bind
43111	1	10103	7	11	NULL	NULL	NULL	CRP	GP		bind					E-LDL	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2348_s_143	10521363	A dose-dependent inhibition of CRP binding to E-LDL was observed, indicating that CRP interacted with its classical ligand 25 26  within the degraded LDL particles.	bind
43112	2	10103	7	11	NULL	NULL	NULL	CRP	GP		interacts with					classical ligand	Chemical				NULL	degraded LDL particles	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2348_s_143	10521363	A dose-dependent inhibition of CRP binding to E-LDL was observed, indicating that CRP interacted with its classical ligand 25 26  within the degraded LDL particles.	bind
35372	1	10104	6	11	NULL	NULL	NULL	sMT1	Chemical		bind					M4 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_63_1_26_s_170	12488533	A dose-dependent inhibition was also observed for the binding of sMT1 to the M4 receptor with an IC50 of 5.5 muM.	bind
43114	1	10104	7	11	NULL	NULL	NULL	sMT1	Chemical		bind					M4 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_63_1_26_s_170	12488533	A dose-dependent inhibition was also observed for the binding of sMT1 to the M4 receptor with an IC50 of 5.5 muM.	bind
35373	1	10105	6	11	NULL	NULL	NULL	ScKar2p	GP		bind					GST-63Jp	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_18_6923_s_355	10958688	A dose-dependent stimulation of  ScKar2p binding to GST-63Jp was observed (Fig.  7), and a significant amount of  ScSls1p remained bound to the glutathione pellet.	bind
43115	1	10105	7	11	NULL	NULL	NULL	ScKar2p	GP		bind					GST-63Jp	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_18_6923_s_355	10958688	A dose-dependent stimulation of  ScKar2p binding to GST-63Jp was observed (Fig.  7), and a significant amount of  ScSls1p remained bound to the glutathione pellet.	bind
35374	1	10106	6	11	NULL	NULL	NULL	NAP	GP		bind					tubulin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_27_28531_s_101	15123709	A dot blot assay performed with spotted tubulin indicated NAP binding to tubulin ( Fig. 2 B).	bind
43117	1	10106	7	11	NULL	NULL	NULL	NAP	GP		bind					tubulin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_27_28531_s_101	15123709	A dot blot assay performed with spotted tubulin indicated NAP binding to tubulin ( Fig. 2 B).	bind
35375	1	10107	6	11	NULL	NULL	NULL	fibronectin	GP		bind					chlamydial EB	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3935_s_40	12065538	A dot blot assay was used to test binding of fibronectin to chlamydial EB.	bind
43118	1	10107	7	11	NULL	NULL	NULL	fibronectin	GP		bind					chlamydial EB	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_7_3935_s_40	12065538	A dot blot assay was used to test binding of fibronectin to chlamydial EB.	bind
35376	1	10108	6	11	NULL	NULL	NULL	RhoG	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_nature_424_6947_461_s_41	12879077	A dot-blot assay using GTP-gammaS- or GDP-loaded purified GST RhoG as a probe showed that the GTP-bound form of RhoG  directly interacted with Elmo ( Fig. 1c).	bind
35377	2	10108	6	11	NULL	NULL	NULL	statement 1	GP		interacts with		directly			Elmo	GP				NULL		NULL	NULL	NULL	NULL	gw70_nature_424_6947_461_s_41	12879077	A dot-blot assay using GTP-gammaS- or GDP-loaded purified GST RhoG as a probe showed that the GTP-bound form of RhoG  directly interacted with Elmo ( Fig. 1c).	bind
43119	1	10108	7	11	NULL	NULL	NULL	RhoG	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_nature_424_6947_461_s_41	12879077	A dot-blot assay using GTP-gammaS- or GDP-loaded purified GST RhoG as a probe showed that the GTP-bound form of RhoG  directly interacted with Elmo ( Fig. 1c).	bind
43120	2	10108	7	11	NULL	NULL	NULL	statement 1	GP		interacts with		directly			Elmo	GP				NULL		NULL	NULL	NULL	NULL	gw70_nature_424_6947_461_s_41	12879077	A dot-blot assay using GTP-gammaS- or GDP-loaded purified GST RhoG as a probe showed that the GTP-bound form of RhoG  directly interacted with Elmo ( Fig. 1c).	bind
35378	1	10109	6	11	NULL	NULL	NULL	Cdk2	GP		bind		indirectly			p21	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_32_29282_s_139	15964852	A double deletion mutant lacking the CDK-binding site and cy1 (p21 deltacy1, CDK) could also bind Cdk2 NFG, indicating that indirect binding of Cdk2 to p21 does not absolutely require cy1.	bind
35379	2	10109	6	11	NULL	NULL	NULL	statement 1	Process		does not require					cy1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_32_29282_s_139	15964852	A double deletion mutant lacking the CDK-binding site and cy1 (p21 deltacy1, CDK) could also bind Cdk2 NFG, indicating that indirect binding of Cdk2 to p21 does not absolutely require cy1.	bind
35380	3	10109	6	11	NULL	NULL	NULL	p21 deltacy1, CDK	GP	double deletion mutant	lacks								\tCDK-binding site;;CDK		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_32_29282_s_139	15964852	A double deletion mutant lacking the CDK-binding site and cy1 (p21 deltacy1, CDK) could also bind Cdk2 NFG, indicating that indirect binding of Cdk2 to p21 does not absolutely require cy1.	bind
35381	4	10109	6	11	NULL	NULL	NULL	p21 deltacy1, CDK	GP	double deletion mutant	bind					Cdk2 NFG	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_32_29282_s_139	15964852	A double deletion mutant lacking the CDK-binding site and cy1 (p21 deltacy1, CDK) could also bind Cdk2 NFG, indicating that indirect binding of Cdk2 to p21 does not absolutely require cy1.	bind
57320	5	10109	6	11	NULL	NULL	NULL	statement 4	Process		indicates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_32_29282_s_139	15964852	A double deletion mutant lacking the CDK-binding site and cy1 (p21 deltacy1, CDK) could also bind Cdk2 NFG, indicating that indirect binding of Cdk2 to p21 does not absolutely require cy1.	bind
43121	1	10109	7	11	NULL	NULL	NULL	Cdk2	GP		bind		indirectly			p21	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_32_29282_s_139	15964852	A double deletion mutant lacking the CDK-binding site and cy1 (p21 deltacy1, CDK) could also bind Cdk2 NFG, indicating that indirect binding of Cdk2 to p21 does not absolutely require cy1.	bind
43122	2	10109	7	11	NULL	NULL	NULL	statement 1	Process		does not require					cy1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_32_29282_s_139	15964852	A double deletion mutant lacking the CDK-binding site and cy1 (p21 deltacy1, CDK) could also bind Cdk2 NFG, indicating that indirect binding of Cdk2 to p21 does not absolutely require cy1.	bind
43123	3	10109	7	11	NULL	NULL	NULL	p21 deltacy1, CDK	GP	double deletion mutant	lacks								CDK-binding site;;CDK		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_32_29282_s_139	15964852	A double deletion mutant lacking the CDK-binding site and cy1 (p21 deltacy1, CDK) could also bind Cdk2 NFG, indicating that indirect binding of Cdk2 to p21 does not absolutely require cy1.	bind
43125	4	10109	7	11	NULL	NULL	NULL	p21 deltacy1, CDK	GP	double deletion mutant	bind					Cdk2 NFG	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_32_29282_s_139	15964852	A double deletion mutant lacking the CDK-binding site and cy1 (p21 deltacy1, CDK) could also bind Cdk2 NFG, indicating that indirect binding of Cdk2 to p21 does not absolutely require cy1.	bind
57321	5	10109	7	11	NULL	NULL	NULL	statement 4	Process		indicates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_32_29282_s_139	15964852	A double deletion mutant lacking the CDK-binding site and cy1 (p21 deltacy1, CDK) could also bind Cdk2 NFG, indicating that indirect binding of Cdk2 to p21 does not absolutely require cy1.	bind
35633	1	10110	6	11	NULL	NULL	NULL	Id3/1	GP		is replaced by			aspartic acid		Id1	GP		tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_19785_s_190	9242638	A double mutant (Fig.  6,  line 11), created by altering the aspartic acid and histidine residues of Id3/1 to the complementary tyrosine and glycine residues of Id1, resulted in almost full binding to MyoD, increased binding to Myf-5, and weak binding to MRF4/Myf-6.	bind
35634	2	10110	6	11	NULL	NULL	NULL	Id3/1	GP		is replaced by			histidine		Id1	GP		glycine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_19785_s_190	9242638	A double mutant (Fig.  6,  line 11), created by altering the aspartic acid and histidine residues of Id3/1 to the complementary tyrosine and glycine residues of Id1, resulted in almost full binding to MyoD, increased binding to Myf-5, and weak binding to MRF4/Myf-6.	bind
35635	3	10110	6	11	NULL	NULL	NULL	statement 1	Process		occurs simultaneously with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_19785_s_190	9242638	A double mutant (Fig.  6,  line 11), created by altering the aspartic acid and histidine residues of Id3/1 to the complementary tyrosine and glycine residues of Id1, resulted in almost full binding to MyoD, increased binding to Myf-5, and weak binding to MRF4/Myf-6.	bind
35636	4	10110	6	11	NULL	NULL	NULL	Id3/1	GP	double mutant	is created by					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_19785_s_190	9242638	A double mutant (Fig.  6,  line 11), created by altering the aspartic acid and histidine residues of Id3/1 to the complementary tyrosine and glycine residues of Id1, resulted in almost full binding to MyoD, increased binding to Myf-5, and weak binding to MRF4/Myf-6.	bind
35637	5	10110	6	11	NULL	NULL	NULL	Id3/1	GP	double mutant	bind					MyoD	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_19785_s_190	9242638	A double mutant (Fig.  6,  line 11), created by altering the aspartic acid and histidine residues of Id3/1 to the complementary tyrosine and glycine residues of Id1, resulted in almost full binding to MyoD, increased binding to Myf-5, and weak binding to MRF4/Myf-6.	bind
35638	6	10110	6	11	NULL	NULL	NULL	Id3/1	GP	double mutant	bind		increased			Myf5	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_19785_s_190	9242638	A double mutant (Fig.  6,  line 11), created by altering the aspartic acid and histidine residues of Id3/1 to the complementary tyrosine and glycine residues of Id1, resulted in almost full binding to MyoD, increased binding to Myf-5, and weak binding to MRF4/Myf-6.	bind
35639	7	10110	6	11	NULL	NULL	NULL	Id3/1	GP	double mutant	bind		weak			MRF4/Myf-6	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_19785_s_190	9242638	A double mutant (Fig.  6,  line 11), created by altering the aspartic acid and histidine residues of Id3/1 to the complementary tyrosine and glycine residues of Id1, resulted in almost full binding to MyoD, increased binding to Myf-5, and weak binding to MRF4/Myf-6.	bind
43126	1	10110	7	11	NULL	NULL	NULL	 Id3/1 	GP		is replaced by			aspartic acid residue		Id1	GP		tyrosine  residue		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_19785_s_190	9242638	A double mutant (Fig.  6,  line 11), created by altering the aspartic acid and histidine residues of Id3/1 to the complementary tyrosine and glycine residues of Id1, resulted in almost full binding to MyoD, increased binding to Myf-5, and weak binding to MRF4/Myf-6.	bind
43127	4	10110	7	11	NULL	NULL	NULL	statement 3	Process		creates					Id3/1	GP	double mutant			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_19785_s_190	9242638	A double mutant (Fig.  6,  line 11), created by altering the aspartic acid and histidine residues of Id3/1 to the complementary tyrosine and glycine residues of Id1, resulted in almost full binding to MyoD, increased binding to Myf-5, and weak binding to MRF4/Myf-6.	bind
43129	5	10110	7	11	NULL	NULL	NULL	Id3/1	GP	double mutant	bind					 MyoD	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_19785_s_190	9242638	A double mutant (Fig.  6,  line 11), created by altering the aspartic acid and histidine residues of Id3/1 to the complementary tyrosine and glycine residues of Id1, resulted in almost full binding to MyoD, increased binding to Myf-5, and weak binding to MRF4/Myf-6.	bind
50213	2	10110	7	11	NULL	NULL	NULL	Id3/1	GP		is replaced by			histidine residue		Id1	GP		glycine residue		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_19785_s_190	9242638	A double mutant (Fig.  6,  line 11), created by altering the aspartic acid and histidine residues of Id3/1 to the complementary tyrosine and glycine residues of Id1, resulted in almost full binding to MyoD, increased binding to Myf-5, and weak binding to MRF4/Myf-6.	bind
50214	3	10110	7	11	NULL	NULL	NULL	statement 1	Process		occur simultaneously with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_19785_s_190	9242638	A double mutant (Fig.  6,  line 11), created by altering the aspartic acid and histidine residues of Id3/1 to the complementary tyrosine and glycine residues of Id1, resulted in almost full binding to MyoD, increased binding to Myf-5, and weak binding to MRF4/Myf-6.	bind
50215	6	10110	7	11	NULL	NULL	NULL	Id3/1	GP	double mutant	bind		increased			Myf-5	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_19785_s_190	9242638	A double mutant (Fig.  6,  line 11), created by altering the aspartic acid and histidine residues of Id3/1 to the complementary tyrosine and glycine residues of Id1, resulted in almost full binding to MyoD, increased binding to Myf-5, and weak binding to MRF4/Myf-6.	bind
50216	7	10110	7	11	NULL	NULL	NULL	Id3/1	GP	double mutant	bind		weakly			MRF4/Myf-6	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_19785_s_190	9242638	A double mutant (Fig.  6,  line 11), created by altering the aspartic acid and histidine residues of Id3/1 to the complementary tyrosine and glycine residues of Id1, resulted in almost full binding to MyoD, increased binding to Myf-5, and weak binding to MRF4/Myf-6.	bind
35382	1	10111	6	11	NULL	NULL	NULL			double mutant	bind			D150K;; D182K		Cu(I)	Chemical	wild type			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_40_34113_s_214	16091356	A double mutant containing D150K and D182K substitutions was purified and found to exhibit wild type Cu(I) and Cu(II) binding and was not further pursued (data not shown).	bind
35383	2	10111	6	11	NULL	NULL	NULL			double mutant	bind			D150K;; D182K		Cu(II)	Chemical	wild type			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_40_34113_s_214	16091356	A double mutant containing D150K and D182K substitutions was purified and found to exhibit wild type Cu(I) and Cu(II) binding and was not further pursued (data not shown).	bind
43130	1	10111	7	11	NULL	NULL	NULL			double mutant	bind			D150K;;D182K		 Cu(I)	Chemical	wild type			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_40_34113_s_214	16091356	A double mutant containing D150K and D182K substitutions was purified and found to exhibit wild type Cu(I) and Cu(II) binding and was not further pursued (data not shown).	bind
43131	2	10111	7	11	NULL	NULL	NULL			double mutant	bind			D150K;; D182K		Cu(II)	Chemical	wild type			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_40_34113_s_214	16091356	A double mutant containing D150K and D182K substitutions was purified and found to exhibit wild type Cu(I) and Cu(II) binding and was not further pursued (data not shown).	bind
43135	1	10112	7	10	NULL	0	NULL	fnbA genes	NULL	S. aureus	is required for	NULL				fibronectin 	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_13_3999_s_200	11395464	A double mutant of  S. aureus lacking both genes for fibronectin binding ( fnbA and  fnbB) was constructed ( 5).	bind
43136	2	10112	7	10	NULL	0	NULL	fnbB genes	NULL	S. aureus	is required for	NULL				fibronectin	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_13_3999_s_200	11395464	A double mutant of  S. aureus lacking both genes for fibronectin binding ( fnbA and  fnbB) was constructed ( 5).	bind
35384	1	10113	6	11	NULL	NULL	NULL	E6	GP		bind					BRCA1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_39_33165_s_187	15983032	A double point mutation that disrupts both zinc finger domains of E6-(C66,136G) abrogated the binding of E6 to BRCA1.	bind
35385	3	10113	6	11	NULL	NULL	NULL	statement 2	Process		abrogates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_39_33165_s_187	15983032	A double point mutation that disrupts both zinc finger domains of E6-(C66,136G) abrogated the binding of E6 to BRCA1.	bind
49557	2	10113	6	11	NULL	NULL	NULL			double point mutation	disrupts					E6	GP		\tzinc finger domains C66,136G		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_39_33165_s_187	15983032	A double point mutation that disrupts both zinc finger domains of E6-(C66,136G) abrogated the binding of E6 to BRCA1.	bind
43137	1	10113	7	11	NULL	NULL	NULL	E6 	GP		bind					BRCA1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_39_33165_s_187	15983032	A double point mutation that disrupts both zinc finger domains of E6-(C66,136G) abrogated the binding of E6 to BRCA1.	bind
43138	2	10113	7	11	NULL	NULL	NULL			double point mutation	disrupts					E6	GP		zinc finger domains C66,136G		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_39_33165_s_187	15983032	A double point mutation that disrupts both zinc finger domains of E6-(C66,136G) abrogated the binding of E6 to BRCA1.	bind
43139	3	10113	7	11	NULL	NULL	NULL	statement 2	Process		abrogates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_39_33165_s_187	15983032	A double point mutation that disrupts both zinc finger domains of E6-(C66,136G) abrogated the binding of E6 to BRCA1.	bind
35387	1	10114	6	11	NULL	NULL	NULL	IF2	GP		bind					fAA-tRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_3_1891_s_117	8999877	A double reciprocal plot of 1/ r, where  r is the fraction of IF2 bound with fAA-tRNA against [1/fAA-tRNA free is shown on Fig.  5.	bind
43140	1	10114	7	11	NULL	NULL	NULL	IF2	GP		bind					 fAA-tRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_3_1891_s_117	8999877	A double reciprocal plot of 1/ r, where  r is the fraction of IF2 bound with fAA-tRNA against [1/fAA-tRNA free is shown on Fig.  5.	bind
35388	1	10115	6	11	NULL	NULL	NULL	fibrinogen	GP		bind								G708N		NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_53	12730600	A double reciprocal plot of fibrinogen binding to G708N revealed a dissociation constant ( Kd) of 180 nM, similar to the  Kd's of 81 nM and 178 nM for fibrinogen binding to ADP-stimulated and epinephrine-stimulated platelets, respectively (  20).	bind
35389	4	10115	6	11	NULL	NULL	NULL	fibrinogen	GP		bind					statement 2	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_53	12730600	A double reciprocal plot of fibrinogen binding to G708N revealed a dissociation constant ( Kd) of 180 nM, similar to the  Kd's of 81 nM and 178 nM for fibrinogen binding to ADP-stimulated and epinephrine-stimulated platelets, respectively (  20).	bind
35390	5	10115	6	11	NULL	NULL	NULL	fibrinogen	GP		bind					statement 3	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_53	12730600	A double reciprocal plot of fibrinogen binding to G708N revealed a dissociation constant ( Kd) of 180 nM, similar to the  Kd's of 81 nM and 178 nM for fibrinogen binding to ADP-stimulated and epinephrine-stimulated platelets, respectively (  20).	bind
49583	2	10115	6	11	NULL	NULL	NULL	platelets	OrganismPart		is stimulated by					ADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_53	12730600	A double reciprocal plot of fibrinogen binding to G708N revealed a dissociation constant ( Kd) of 180 nM, similar to the  Kd's of 81 nM and 178 nM for fibrinogen binding to ADP-stimulated and epinephrine-stimulated platelets, respectively (  20).	bind
49584	3	10115	6	11	NULL	NULL	NULL	platelets	OrganismPart		is stimulated by					epinephrine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_53	12730600	A double reciprocal plot of fibrinogen binding to G708N revealed a dissociation constant ( Kd) of 180 nM, similar to the  Kd's of 81 nM and 178 nM for fibrinogen binding to ADP-stimulated and epinephrine-stimulated platelets, respectively (  20).	bind
43141	1	10115	7	11	NULL	NULL	NULL	fibrinogen	GP		bind								G708N		NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_53	12730600	A double reciprocal plot of fibrinogen binding to G708N revealed a dissociation constant ( Kd) of 180 nM, similar to the  Kd's of 81 nM and 178 nM for fibrinogen binding to ADP-stimulated and epinephrine-stimulated platelets, respectively (  20).	bind
43142	2	10115	7	11	NULL	NULL	NULL	platelets	OrganismPart		is stimulated by					ADP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_53	12730600	A double reciprocal plot of fibrinogen binding to G708N revealed a dissociation constant ( Kd) of 180 nM, similar to the  Kd's of 81 nM and 178 nM for fibrinogen binding to ADP-stimulated and epinephrine-stimulated platelets, respectively (  20).	bind
43143	3	10115	7	11	NULL	NULL	NULL	platelets	OrganismPart		is stimulated by					epinephrine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_53	12730600	A double reciprocal plot of fibrinogen binding to G708N revealed a dissociation constant ( Kd) of 180 nM, similar to the  Kd's of 81 nM and 178 nM for fibrinogen binding to ADP-stimulated and epinephrine-stimulated platelets, respectively (  20).	bind
43144	4	10115	7	11	NULL	NULL	NULL	statement 2	OrganismPart		binds					fibrinogen	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_53	12730600	A double reciprocal plot of fibrinogen binding to G708N revealed a dissociation constant ( Kd) of 180 nM, similar to the  Kd's of 81 nM and 178 nM for fibrinogen binding to ADP-stimulated and epinephrine-stimulated platelets, respectively (  20).	bind
43145	5	10115	7	11	NULL	NULL	NULL	statement 3	OrganismPart		binds					fibrinogen	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_300_5620_795_s_53	12730600	A double reciprocal plot of fibrinogen binding to G708N revealed a dissociation constant ( Kd) of 180 nM, similar to the  Kd's of 81 nM and 178 nM for fibrinogen binding to ADP-stimulated and epinephrine-stimulated platelets, respectively (  20).	bind
35391	1	10116	6	11	NULL	NULL	NULL	K88ab adhesin	GP		bind					pSTf	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2336_s_110	11953368	A double-reciprocal plot of this binding data was used to determine that the dissociation constant for the binding of K88ab adhesin to pSTf is 75 muM.	bind
43146	1	10116	7	11	NULL	NULL	NULL	K88ab adhesin	GP		bind					pSTf	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2336_s_110	11953368	A double-reciprocal plot of this binding data was used to determine that the dissociation constant for the binding of K88ab adhesin to pSTf is 75 muM.	bind
35392	1	10118	6	11	NULL	NULL	NULL	HOXC11	GP		bind					CE-LPH1-24 probe	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_13297_s_150	9582375	A double-stranded oligonucleotide covering this vector sequence, referred to as BSK-17 in Fig.  1, was able to compete for HOXC11 binding to the CE-LPH1-24 probe in EMSA analysis (Fig.  5,  lane 9).	bind
49588	2	10118	6	11	NULL	NULL	NULL	BSK-17	GP		bind					HOXC11	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_13297_s_150	9582375	A double-stranded oligonucleotide covering this vector sequence, referred to as BSK-17 in Fig.  1, was able to compete for HOXC11 binding to the CE-LPH1-24 probe in EMSA analysis (Fig.  5,  lane 9).	bind
49589	3	10118	6	11	NULL	NULL	NULL	statement 2	Process		competes with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_13297_s_150	9582375	A double-stranded oligonucleotide covering this vector sequence, referred to as BSK-17 in Fig.  1, was able to compete for HOXC11 binding to the CE-LPH1-24 probe in EMSA analysis (Fig.  5,  lane 9).	bind
43147	1	10118	7	11	NULL	NULL	NULL	 HOXC11	GP		bind					CE-LPH1-24 probe	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_13297_s_150	9582375	A double-stranded oligonucleotide covering this vector sequence, referred to as BSK-17 in Fig.  1, was able to compete for HOXC11 binding to the CE-LPH1-24 probe in EMSA analysis (Fig.  5,  lane 9).	bind
43148	2	10118	7	11	NULL	NULL	NULL	BSK-17	GP		bind					HOXC11	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_13297_s_150	9582375	A double-stranded oligonucleotide covering this vector sequence, referred to as BSK-17 in Fig.  1, was able to compete for HOXC11 binding to the CE-LPH1-24 probe in EMSA analysis (Fig.  5,  lane 9).	bind
49587	3	10118	7	11	NULL	NULL	NULL	statement 2	Process		competes with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_13297_s_150	9582375	A double-stranded oligonucleotide covering this vector sequence, referred to as BSK-17 in Fig.  1, was able to compete for HOXC11 binding to the CE-LPH1-24 probe in EMSA analysis (Fig.  5,  lane 9).	bind
35393	1	10120	6	11	NULL	NULL	NULL	U11	GP		bind		efficiently			NRS	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_37_38201_s_154	15252020	A downstream G-rich region is required for efficient U11 binding to the NRS.	bind
35394	2	10120	6	11	NULL	NULL	NULL				is required for				G-rich region	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_37_38201_s_154	15252020	A downstream G-rich region is required for efficient U11 binding to the NRS.	bind
43149	1	10120	7	11	NULL	NULL	NULL	U11	GP		bind					NRS	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_37_38201_s_154	15252020	A downstream G-rich region is required for efficient U11 binding to the NRS.	bind
43150	2	10120	7	11	NULL	NULL	NULL				is required for				G-rich region	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_37_38201_s_154	15252020	A downstream G-rich region is required for efficient U11 binding to the NRS.	bind
35395	1	10121	6	11	NULL	NULL	NULL	atf1/gad7 genes	GP		encodes for					heterodimeric bZIP transcriptional activator	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6426_s_28	10938120	A downstream target of the MAPK, a heterodimeric bZIP transcriptional activator encoded by the  atf1/gad7 and the  pcr1 genes, is required to derepress  fbp1 transcription ( 22,  50,  55,  63).	bind
35396	2	10121	6	11	NULL	NULL	NULL	pcr1 gene	GP		encodes for					heterodimeric bZIP transcriptional activator	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6426_s_28	10938120	A downstream target of the MAPK, a heterodimeric bZIP transcriptional activator encoded by the  atf1/gad7 and the  pcr1 genes, is required to derepress  fbp1 transcription ( 22,  50,  55,  63).	bind
35397	3	10121	6	11	NULL	NULL	NULL	downstream target of the MAPK	GP		is a type of					heterodimeric bZIP transcriptional activator	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6426_s_28	10938120	A downstream target of the MAPK, a heterodimeric bZIP transcriptional activator encoded by the  atf1/gad7 and the  pcr1 genes, is required to derepress  fbp1 transcription ( 22,  50,  55,  63).	bind
35398	4	10121	6	11	NULL	NULL	NULL	downstream target of the MAPK	GP		derepress					fbp1	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6426_s_28	10938120	A downstream target of the MAPK, a heterodimeric bZIP transcriptional activator encoded by the  atf1/gad7 and the  pcr1 genes, is required to derepress  fbp1 transcription ( 22,  50,  55,  63).	bind
43151	1	10121	7	11	NULL	NULL	NULL	atf1/gad7 genes	GP		encodes					MAPK	GP	downstream target of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6426_s_28	10938120	A downstream target of the MAPK, a heterodimeric bZIP transcriptional activator encoded by the  atf1/gad7 and the  pcr1 genes, is required to derepress  fbp1 transcription ( 22,  50,  55,  63).	bind
43152	2	10121	7	11	NULL	NULL	NULL	pcr1 genes	GP		encodes					MAPK	GP	downstream target of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6426_s_28	10938120	A downstream target of the MAPK, a heterodimeric bZIP transcriptional activator encoded by the  atf1/gad7 and the  pcr1 genes, is required to derepress  fbp1 transcription ( 22,  50,  55,  63).	bind
43153	3	10121	7	11	NULL	NULL	NULL	downstream target of MAPK	GP		is a type of					heterodimeric bZIP transcriptional activator	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6426_s_28	10938120	A downstream target of the MAPK, a heterodimeric bZIP transcriptional activator encoded by the  atf1/gad7 and the  pcr1 genes, is required to derepress  fbp1 transcription ( 22,  50,  55,  63).	bind
43154	4	10121	7	11	NULL	NULL	NULL	downstream target of MAPK	GP		derepress					fbp1	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6426_s_28	10938120	A downstream target of the MAPK, a heterodimeric bZIP transcriptional activator encoded by the  atf1/gad7 and the  pcr1 genes, is required to derepress  fbp1 transcription ( 22,  50,  55,  63).	bind
35399	1	10122	6	11	NULL	NULL	NULL	DR-1	GP		bind					HNF-4	GP				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_44_4_686_s_187	12562861	A DR-1 also binds HNF-4 ( ).	bind
43155	1	10122	7	11	NULL	NULL	NULL	 DR-1	GP		binds					HNF-4 	GP				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_44_4_686_s_187	12562861	A DR-1 also binds HNF-4 ( ).	bind
35400	1	10124	6	11	NULL	NULL	NULL	ezrin	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_867_s_328	11238445	A dramatic increase in ezrin binding to actin suggests that ezrin is likely to be the PIP2 regulator of membrane - cytoskeletal linkage.	bind
35401	2	10124	6	11	NULL	NULL	NULL	ezrin	GP		is 					membrane - cytoskeletal linkage	CellComponent	PIP2 regulator of 			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_867_s_328	11238445	A dramatic increase in ezrin binding to actin suggests that ezrin is likely to be the PIP2 regulator of membrane - cytoskeletal linkage.	bind
35402	3	10124	6	11	NULL	NULL	NULL	statement 1	Process	increase in	suggests					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_867_s_328	11238445	A dramatic increase in ezrin binding to actin suggests that ezrin is likely to be the PIP2 regulator of membrane - cytoskeletal linkage.	bind
43156	1	10124	7	11	NULL	NULL	NULL	ezrin	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_867_s_328	11238445	A dramatic increase in ezrin binding to actin suggests that ezrin is likely to be the PIP2 regulator of membrane - cytoskeletal linkage.	bind
43157	2	10124	7	11	NULL	NULL	NULL	ezrin	GP		likey to be the					membrane - cytoskeletal linkage	CellComponent	PIP2 regulator of 			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_5_867_s_328	11238445	A dramatic increase in ezrin binding to actin suggests that ezrin is likely to be the PIP2 regulator of membrane - cytoskeletal linkage.	bind
35640	1	10126	6	11	NULL	NULL	NULL	BUDeR	Chemical		inhibits					AP1-like	GP				NULL	HEK cell line	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_13_8630_s_187	10085100	A dramatic inhibition of  cis-acting transcription factor AP1-like-, gamma-interferon activation sequence-, and especially NF-kappaB-DNA binding by the GCs DEX and BUDeR, temporally correlating to a reduction in cyclooxygenase-2 message synthesis, has recently been demonstrated in HEK cell lines ( 14).	bind
35641	2	10126	6	11	NULL	NULL	NULL	BUDeR	Chemical		inhibits					gamma-interferon activation sequence-	NucleicAcid				NULL	HEK cell line	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_13_8630_s_187	10085100	A dramatic inhibition of  cis-acting transcription factor AP1-like-, gamma-interferon activation sequence-, and especially NF-kappaB-DNA binding by the GCs DEX and BUDeR, temporally correlating to a reduction in cyclooxygenase-2 message synthesis, has recently been demonstrated in HEK cell lines ( 14).	bind
35642	3	10126	6	11	NULL	NULL	NULL	NF-kappaB	GP		bind					DNA	NucleicAcid				NULL	HEK cell line	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_13_8630_s_187	10085100	A dramatic inhibition of  cis-acting transcription factor AP1-like-, gamma-interferon activation sequence-, and especially NF-kappaB-DNA binding by the GCs DEX and BUDeR, temporally correlating to a reduction in cyclooxygenase-2 message synthesis, has recently been demonstrated in HEK cell lines ( 14).	bind
35643	4	10126	6	11	NULL	NULL	NULL	BUDeR	Chemical		inhibits					statement 3	Process				NULL	HEK cell line	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_13_8630_s_187	10085100	A dramatic inhibition of  cis-acting transcription factor AP1-like-, gamma-interferon activation sequence-, and especially NF-kappaB-DNA binding by the GCs DEX and BUDeR, temporally correlating to a reduction in cyclooxygenase-2 message synthesis, has recently been demonstrated in HEK cell lines ( 14).	bind
35644	5	10126	6	11	NULL	NULL	NULL	GCs DEX	Chemical		inhibits					AP1-like	GP				NULL	HEK cell line	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_13_8630_s_187	10085100	A dramatic inhibition of  cis-acting transcription factor AP1-like-, gamma-interferon activation sequence-, and especially NF-kappaB-DNA binding by the GCs DEX and BUDeR, temporally correlating to a reduction in cyclooxygenase-2 message synthesis, has recently been demonstrated in HEK cell lines ( 14).	bind
35645	6	10126	6	11	NULL	NULL	NULL	GCs DEX	Chemical		inhibits					gamma-interferon activation sequence	NucleicAcid				NULL	HEK cell line	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_13_8630_s_187	10085100	A dramatic inhibition of  cis-acting transcription factor AP1-like-, gamma-interferon activation sequence-, and especially NF-kappaB-DNA binding by the GCs DEX and BUDeR, temporally correlating to a reduction in cyclooxygenase-2 message synthesis, has recently been demonstrated in HEK cell lines ( 14).	bind
35646	7	10126	6	11	NULL	NULL	NULL	GCs DEX	Chemical		inhibits					statement 3	Process				NULL	HEK cell line	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_13_8630_s_187	10085100	A dramatic inhibition of  cis-acting transcription factor AP1-like-, gamma-interferon activation sequence-, and especially NF-kappaB-DNA binding by the GCs DEX and BUDeR, temporally correlating to a reduction in cyclooxygenase-2 message synthesis, has recently been demonstrated in HEK cell lines ( 14).	bind
35647	8	10126	6	11	NULL	NULL	NULL	AP1	GP		is a type of					cis-acting transcription factor	GP				NULL	HEK cell line	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_13_8630_s_187	10085100	A dramatic inhibition of  cis-acting transcription factor AP1-like-, gamma-interferon activation sequence-, and especially NF-kappaB-DNA binding by the GCs DEX and BUDeR, temporally correlating to a reduction in cyclooxygenase-2 message synthesis, has recently been demonstrated in HEK cell lines ( 14).	bind
43268	1	10126	7	11	NULL	NULL	NULL	NF-kappaB	GP		bind					DNA	NucleicAcid				NULL	HEK cell lines	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_13_8630_s_187	10085100	A dramatic inhibition of  cis-acting transcription factor AP1-like-, gamma-interferon activation sequence-, and especially NF-kappaB-DNA binding by the GCs DEX and BUDeR, temporally correlating to a reduction in cyclooxygenase-2 message synthesis, has recently been demonstrated in HEK cell lines ( 14).	bind
43286	2	10126	7	11	NULL	NULL	NULL	GCs DEX	Chemical		inhibit					statement 1	Process				NULL	HEK cell lines	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_13_8630_s_187	10085100	A dramatic inhibition of  cis-acting transcription factor AP1-like-, gamma-interferon activation sequence-, and especially NF-kappaB-DNA binding by the GCs DEX and BUDeR, temporally correlating to a reduction in cyclooxygenase-2 message synthesis, has recently been demonstrated in HEK cell lines ( 14).	bind
43287	3	10126	7	11	NULL	NULL	NULL	BUDeR	Chemical		inhibit					statement 1	Process				NULL	HEK cell lines	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_13_8630_s_187	10085100	A dramatic inhibition of  cis-acting transcription factor AP1-like-, gamma-interferon activation sequence-, and especially NF-kappaB-DNA binding by the GCs DEX and BUDeR, temporally correlating to a reduction in cyclooxygenase-2 message synthesis, has recently been demonstrated in HEK cell lines ( 14).	bind
43288	4	10126	7	11	NULL	NULL	NULL	statement 2	Process		correlates to		temporally			cyclooxygenase-2 message 	GP	reduction of;;synthesis of			NULL	HEK cell lines	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_13_8630_s_187	10085100	A dramatic inhibition of  cis-acting transcription factor AP1-like-, gamma-interferon activation sequence-, and especially NF-kappaB-DNA binding by the GCs DEX and BUDeR, temporally correlating to a reduction in cyclooxygenase-2 message synthesis, has recently been demonstrated in HEK cell lines ( 14).	bind
43289	5	10126	7	11	NULL	NULL	NULL	statement 3	Process		correlates to		temporally			cyclooxygenase-2 message 	GP	reduction of;;synthesis of			NULL	HEK cell lines	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_13_8630_s_187	10085100	A dramatic inhibition of  cis-acting transcription factor AP1-like-, gamma-interferon activation sequence-, and especially NF-kappaB-DNA binding by the GCs DEX and BUDeR, temporally correlating to a reduction in cyclooxygenase-2 message synthesis, has recently been demonstrated in HEK cell lines ( 14).	bind
35648	1	10127	6	11	NULL	NULL	NULL	fusion protein	GP		contains					hCLCA2	GP		beta4-binding motif		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49406_s_45	14512419	A dramatic inhibition of metastasis of MDA-MB-231 breast cancer cells by a fusion protein containing the beta4-binding motif of hCLCA2 further advances the role of the beta4/CLCA adhesion in pulmonary metastasis.	bind
35649	2	10127	6	11	NULL	NULL	NULL	statement 1	Process		inhibits					MDA-MB-231	Cell	metastasis of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49406_s_45	14512419	A dramatic inhibition of metastasis of MDA-MB-231 breast cancer cells by a fusion protein containing the beta4-binding motif of hCLCA2 further advances the role of the beta4/CLCA adhesion in pulmonary metastasis.	bind
35650	3	10127	6	11	NULL	NULL	NULL	MDA-MB-231	Cell		is a type of					breast cancer cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49406_s_45	14512419	A dramatic inhibition of metastasis of MDA-MB-231 breast cancer cells by a fusion protein containing the beta4-binding motif of hCLCA2 further advances the role of the beta4/CLCA adhesion in pulmonary metastasis.	bind
35651	4	10127	6	11	NULL	NULL	NULL	beta4/CLCA	GP	adhesion of	plays a role in					pulmonary metastasis	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49406_s_45	14512419	A dramatic inhibition of metastasis of MDA-MB-231 breast cancer cells by a fusion protein containing the beta4-binding motif of hCLCA2 further advances the role of the beta4/CLCA adhesion in pulmonary metastasis.	bind
43269	1	10127	7	11	NULL	NULL	NULL	fusion protein 	GP		contains					hCLCA2	GP		beta4-binding motif		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49406_s_45	14512419	A dramatic inhibition of metastasis of MDA-MB-231 breast cancer cells by a fusion protein containing the beta4-binding motif of hCLCA2 further advances the role of the beta4/CLCA adhesion in pulmonary metastasis.	bind
43270	2	10127	7	11	NULL	NULL	NULL	statement 1	Process		inhibits					MDA-MB-231	Cell	 metastasis of 			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49406_s_45	14512419	A dramatic inhibition of metastasis of MDA-MB-231 breast cancer cells by a fusion protein containing the beta4-binding motif of hCLCA2 further advances the role of the beta4/CLCA adhesion in pulmonary metastasis.	bind
43273	3	10127	7	11	NULL	NULL	NULL	beta4/CLCA 	GP	adhesion of	plays a role in					pulmonary metastasis	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49406_s_45	14512419	A dramatic inhibition of metastasis of MDA-MB-231 breast cancer cells by a fusion protein containing the beta4-binding motif of hCLCA2 further advances the role of the beta4/CLCA adhesion in pulmonary metastasis.	bind
49592	4	10127	7	11	NULL	NULL	NULL	MDA-MB-231	Cell		is a type of					breast cancer cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49406_s_45	14512419	A dramatic inhibition of metastasis of MDA-MB-231 breast cancer cells by a fusion protein containing the beta4-binding motif of hCLCA2 further advances the role of the beta4/CLCA adhesion in pulmonary metastasis.	bind
35403	1	10128	6	11	NULL	NULL	NULL	MLCK-FIP	GP		bind					calmodulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_156_3_543_s_91	11815633	A dramatic loss of FRET was seen immediately after ionomycin treatment ( Fig. 2 B), indicated by a shift from red to green or blue, showing that MLCK-FIP bound calmodulin and was therefore activated.	bind
49595	2	10128	6	11	NULL	NULL	NULL	statement 1	Process		activates					MLCK-FIP	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_156_3_543_s_91	11815633	A dramatic loss of FRET was seen immediately after ionomycin treatment ( Fig. 2 B), indicated by a shift from red to green or blue, showing that MLCK-FIP bound calmodulin and was therefore activated.	bind
43293	1	10128	7	11	NULL	NULL	NULL	MLCK-FIP	GP		bind					calmodulin 	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_156_3_543_s_91	11815633	A dramatic loss of FRET was seen immediately after ionomycin treatment ( Fig. 2 B), indicated by a shift from red to green or blue, showing that MLCK-FIP bound calmodulin and was therefore activated.	bind
43294	2	10128	7	11	NULL	NULL	NULL	statement 1	GP		activates					MLCK-FIP 	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_156_3_543_s_91	11815633	A dramatic loss of FRET was seen immediately after ionomycin treatment ( Fig. 2 B), indicated by a shift from red to green or blue, showing that MLCK-FIP bound calmodulin and was therefore activated.	bind
35775	1	10130	6	11	NULL	NULL	NULL	GATA factor family member	GP	Drosophila	bind					Adh	GP			regulatory sequences	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_5_2901_s_369	9566909	A Drosophila GATA factor family member that binds to Adh regulatory sequences is expressed in the developing fat body.	bind
35776	2	10130	6	11	NULL	NULL	NULL	GATA family member	GP	Drosophila	is expressed in					developing fat body	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_5_2901_s_369	9566909	A Drosophila GATA factor family member that binds to Adh regulatory sequences is expressed in the developing fat body.	bind
43295	1	10130	7	11	NULL	NULL	NULL	GATA factor family	GP	Drosophila	bind					Adh	GP			regulatory sequences	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_5_2901_s_369	9566909	A Drosophila GATA factor family member that binds to Adh regulatory sequences is expressed in the developing fat body.	bind
43296	2	10130	7	11	NULL	NULL	NULL	statement 1	GP		is expressed in					developing fat body	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_5_2901_s_369	9566909	A Drosophila GATA factor family member that binds to Adh regulatory sequences is expressed in the developing fat body.	bind
35777	1	10132	6	11	NULL	NULL	NULL	adenomatous polyposis coli	GP	Drosophila homolog	downregulates					beta-catenin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_2_311_s_156	11057903	A Drosophila homolog of the tumor suppressor gene adenomatous polyposis coli down-regulates beta-catenin but its zygotic expression is not essential for the regulation of Armadillo.	bind
35778	2	10132	6	11	NULL	NULL	NULL	adenomatous polyposis coli	Organism		is a type of					tumor suppressor gene	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_2_311_s_156	11057903	A Drosophila homolog of the tumor suppressor gene adenomatous polyposis coli down-regulates beta-catenin but its zygotic expression is not essential for the regulation of Armadillo.	bind
35779	3	10132	6	11	NULL	NULL	NULL	adenomatous polyposis coli	GP	Drosophila homolog;;zygotic expression of	is not essential for					Armadillo	Organism	regulation of			NULL		NULL	NULL	NULL	NULL	gw60_cell_103_2_311_s_156	11057903	A Drosophila homolog of the tumor suppressor gene adenomatous polyposis coli down-regulates beta-catenin but its zygotic expression is not essential for the regulation of Armadillo.	bind
43297	1	10132	7	11	NULL	NULL	NULL	adenomatous polyposis coli	GP	Drosophila homolog of	down-regulates					beta-catenin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_2_311_s_156	11057903	A Drosophila homolog of the tumor suppressor gene adenomatous polyposis coli down-regulates beta-catenin but its zygotic expression is not essential for the regulation of Armadillo.	bind
43298	2	10132	7	11	NULL	NULL	NULL	adenomatous polyposis coli 	GP	zygotic expression of;;Drosophila homolog	is not essential for					Armadillo	Organism	 regulation of			NULL		NULL	NULL	NULL	NULL	gw60_cell_103_2_311_s_156	11057903	A Drosophila homolog of the tumor suppressor gene adenomatous polyposis coli down-regulates beta-catenin but its zygotic expression is not essential for the regulation of Armadillo.	bind
43299	3	10132	7	11	NULL	NULL	NULL	adenomatous polyposis coli	GP		is a type of					 tumor suppressor gene 	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_2_311_s_156	11057903	A Drosophila homolog of the tumor suppressor gene adenomatous polyposis coli down-regulates beta-catenin but its zygotic expression is not essential for the regulation of Armadillo.	bind
35780	1	10133	6	11	NULL	NULL	NULL	TRAF	GP		is					TNF-receptor-associated factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_1_9_s_409	12110163	A Drosophila TNF-receptor-associated factor (TRAF) binds the ste20 kinase Misshapen and activates Jun kinase.	bind
35781	2	10133	6	11	NULL	NULL	NULL	TRAF	GP	Drosophila	bind					misshapen	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_1_9_s_409	12110163	A Drosophila TNF-receptor-associated factor (TRAF) binds the ste20 kinase Misshapen and activates Jun kinase.	bind
35782	3	10133	6	11	NULL	NULL	NULL	Misshapen	GP		is a type of					ste20 kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_1_9_s_409	12110163	A Drosophila TNF-receptor-associated factor (TRAF) binds the ste20 kinase Misshapen and activates Jun kinase.	bind
35783	4	10133	6	11	NULL	NULL	NULL	statement 2	GP		activates					Jun kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_1_9_s_409	12110163	A Drosophila TNF-receptor-associated factor (TRAF) binds the ste20 kinase Misshapen and activates Jun kinase.	bind
43300	1	10133	7	11	NULL	NULL	NULL	TRAF	GP	Drosophila	binds					Misshapen 	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_1_9_s_409	12110163	A Drosophila TNF-receptor-associated factor (TRAF) binds the ste20 kinase Misshapen and activates Jun kinase.	bind
43301	2	10133	7	11	NULL	NULL	NULL	statement 1	GP		activates					Jun kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_1_9_s_409	12110163	A Drosophila TNF-receptor-associated factor (TRAF) binds the ste20 kinase Misshapen and activates Jun kinase.	bind
43302	3	10133	7	11	NULL	NULL	NULL	TRAF	GP		is					TNF-receptor-associated factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_1_9_s_409	12110163	A Drosophila TNF-receptor-associated factor (TRAF) binds the ste20 kinase Misshapen and activates Jun kinase.	bind
49598	4	10133	7	11	NULL	NULL	NULL	Misshapen	GP		is a type of					ste20 kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_1_9_s_409	12110163	A Drosophila TNF-receptor-associated factor (TRAF) binds the ste20 kinase Misshapen and activates Jun kinase.	bind
35784	1	10134	6	11	NULL	NULL	NULL	DSB	NucleicAcid		occurs in					loop DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_18_4075_s_285	12235392	A DSB that occurs in loop DNA is first bound by Ku70/Ku86 that then recruits DNA-PKcs and possibly other proteins to the ends.	bind
35785	2	10134	6	11	NULL	NULL	NULL	DSB	NucleicAcid		bind					Ku70/Ku86	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_18_4075_s_285	12235392	A DSB that occurs in loop DNA is first bound by Ku70/Ku86 that then recruits DNA-PKcs and possibly other proteins to the ends.	bind
36100	3	10134	6	11	NULL	NULL	NULL	DNA-PKcs	NucleicAcid		are recruited to					DNA ends	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_18_4075_s_285	12235392	A DSB that occurs in loop DNA is first bound by Ku70/Ku86 that then recruits DNA-PKcs and possibly other proteins to the ends.	bind
36101	4	10134	6	11	NULL	NULL	NULL	DSB	NucleicAcid		recruits					DNA-PKcs	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_18_4075_s_285	12235392	A DSB that occurs in loop DNA is first bound by Ku70/Ku86 that then recruits DNA-PKcs and possibly other proteins to the ends.	bind
36102	5	10134	6	11	NULL	NULL	NULL	statement 4	Process		occurs after					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_18_4075_s_285	12235392	A DSB that occurs in loop DNA is first bound by Ku70/Ku86 that then recruits DNA-PKcs and possibly other proteins to the ends.	bind
43303	1	10134	7	11	NULL	NULL	NULL	DSB	NucleicAcid		occurs in					loop DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_18_4075_s_285	12235392	A DSB that occurs in loop DNA is first bound by Ku70/Ku86 that then recruits DNA-PKcs and possibly other proteins to the ends.	bind
43304	2	10134	7	11	NULL	NULL	NULL	statement 1	NucleicAcid		bind					Ku70/Ku86	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_18_4075_s_285	12235392	A DSB that occurs in loop DNA is first bound by Ku70/Ku86 that then recruits DNA-PKcs and possibly other proteins to the ends.	bind
43305	3	10134	7	11	NULL	NULL	NULL	statement 2	NucleicAcid		recruits					DNA-PKcs	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_18_4075_s_285	12235392	A DSB that occurs in loop DNA is first bound by Ku70/Ku86 that then recruits DNA-PKcs and possibly other proteins to the ends.	bind
43306	4	10134	7	11	NULL	NULL	NULL	DNA-PKcs \t	NucleicAcid		is recruited to					DNA ends	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_18_4075_s_285	12235392	A DSB that occurs in loop DNA is first bound by Ku70/Ku86 that then recruits DNA-PKcs and possibly other proteins to the ends.	bind
35786	1	10135	6	11	NULL	NULL	NULL	Dazl protein	GP		bind					RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2479_s_4	11410654	A dual approach was taken to understand the RNA-binding specificity of the Dazl protein: (i) traditional SELEX and (ii) a novel tri-hybrid screen.	bind
43307	1	10135	7	11	NULL	NULL	NULL	Dazl protein	GP		bind					RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_12_2479_s_4	11410654	A dual approach was taken to understand the RNA-binding specificity of the Dazl protein: (i) traditional SELEX and (ii) a novel tri-hybrid screen.	bind
35787	1	10136	6	11	NULL	NULL	NULL	FHL2	GP		bind					alpha-integrin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_27_28641_s_358	15117962	A dual binding of FHL2 and FHL3 to both alpha- and beta-integrin chains might provide a stronger connection of the receptor to the cell interior than only a single interaction.	bind
35788	2	10136	6	11	NULL	NULL	NULL	FHL3	GP		bind					alpha-integrin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_27_28641_s_358	15117962	A dual binding of FHL2 and FHL3 to both alpha- and beta-integrin chains might provide a stronger connection of the receptor to the cell interior than only a single interaction.	bind
35789	3	10136	6	11	NULL	NULL	NULL	FHL2			bind					beta-integrin					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_27_28641_s_358	15117962	A dual binding of FHL2 and FHL3 to both alpha- and beta-integrin chains might provide a stronger connection of the receptor to the cell interior than only a single interaction.	bind
35790	4	10136	6	11	NULL	NULL	NULL	FHL3	GP		bind					beta-integrin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_27_28641_s_358	15117962	A dual binding of FHL2 and FHL3 to both alpha- and beta-integrin chains might provide a stronger connection of the receptor to the cell interior than only a single interaction.	bind
43308	1	10136	7	11	NULL	NULL	NULL	FHL2	GP		bind					alpha-integrin chain	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_27_28641_s_358	15117962	A dual binding of FHL2 and FHL3 to both alpha- and beta-integrin chains might provide a stronger connection of the receptor to the cell interior than only a single interaction.	bind
43309	2	10136	7	11	NULL	NULL	NULL	FHL3	GP		bind					beta-integrin chain	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_27_28641_s_358	15117962	A dual binding of FHL2 and FHL3 to both alpha- and beta-integrin chains might provide a stronger connection of the receptor to the cell interior than only a single interaction.	bind
50228	3	10136	7	11	NULL	NULL	NULL	FHL2	GP		bind					beta-integrin chain	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_27_28641_s_358	15117962	A dual binding of FHL2 and FHL3 to both alpha- and beta-integrin chains might provide a stronger connection of the receptor to the cell interior than only a single interaction.	bind
50229	4	10136	7	11	NULL	NULL	NULL	FHL3	GP		bind					alpha-integrin chain	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_27_28641_s_358	15117962	A dual binding of FHL2 and FHL3 to both alpha- and beta-integrin chains might provide a stronger connection of the receptor to the cell interior than only a single interaction.	bind
35791	1	10137	6	11	NULL	NULL	NULL	Id2	GP		is linked to					pRb	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_16_15836_s_20	15691830	A dual connection links Id2 and pRb: when overexpressed, Id2 overrides the tumor suppressor function of RB, allowing binding of E2F to its target genes, promoting entry into S phase and cell proliferation ( ).	bind
35792	2	10137	6	11	NULL	NULL	NULL	Id2	GP	overexpressed	overrides					RB	GP	\ttumor suppressor function of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_16_15836_s_20	15691830	A dual connection links Id2 and pRb: when overexpressed, Id2 overrides the tumor suppressor function of RB, allowing binding of E2F to its target genes, promoting entry into S phase and cell proliferation ( ).	bind
35793	3	10137	6	11	NULL	NULL	NULL	E2F	GP		bind					target genes	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_16_15836_s_20	15691830	A dual connection links Id2 and pRb: when overexpressed, Id2 overrides the tumor suppressor function of RB, allowing binding of E2F to its target genes, promoting entry into S phase and cell proliferation ( ).	bind
35794	4	10137	6	11	NULL	NULL	NULL	statement 2	Process		allows					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_16_15836_s_20	15691830	A dual connection links Id2 and pRb: when overexpressed, Id2 overrides the tumor suppressor function of RB, allowing binding of E2F to its target genes, promoting entry into S phase and cell proliferation ( ).	bind
35795	5	10137	6	11	NULL	NULL	NULL	statement 4	Process		promotes					S phase	Process	entry into			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_16_15836_s_20	15691830	A dual connection links Id2 and pRb: when overexpressed, Id2 overrides the tumor suppressor function of RB, allowing binding of E2F to its target genes, promoting entry into S phase and cell proliferation ( ).	bind
35796	6	10137	6	11	NULL	NULL	NULL	statement 4	Process		promotes					cell	Cell	proliferation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_16_15836_s_20	15691830	A dual connection links Id2 and pRb: when overexpressed, Id2 overrides the tumor suppressor function of RB, allowing binding of E2F to its target genes, promoting entry into S phase and cell proliferation ( ).	bind
43313	1	10137	7	NULL	NULL	0	NULL	 Id2	NULL		links to	NULL				pRb	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_16_15836_s_20	15691830	A dual connection links Id2 and pRb: when overexpressed, Id2 overrides the tumor suppressor function of RB, allowing binding of E2F to its target genes, promoting entry into S phase and cell proliferation ( ).	bind
43314	2	10137	7	NULL	NULL	0	NULL	Id2	NULL	overexpression of	overrides	NULL				RB	NULL	tumor suppressor function of 			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_16_15836_s_20	15691830	A dual connection links Id2 and pRb: when overexpressed, Id2 overrides the tumor suppressor function of RB, allowing binding of E2F to its target genes, promoting entry into S phase and cell proliferation ( ).	bind
43315	3	10137	7	NULL	NULL	0	NULL	E2F	NULL		bind	NULL				target genes	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_16_15836_s_20	15691830	A dual connection links Id2 and pRb: when overexpressed, Id2 overrides the tumor suppressor function of RB, allowing binding of E2F to its target genes, promoting entry into S phase and cell proliferation ( ).	bind
43316	4	10137	7	NULL	NULL	0	NULL	statement 2	NULL		allows	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_16_15836_s_20	15691830	A dual connection links Id2 and pRb: when overexpressed, Id2 overrides the tumor suppressor function of RB, allowing binding of E2F to its target genes, promoting entry into S phase and cell proliferation ( ).	bind
43317	5	10137	7	NULL	NULL	0	NULL	statement 4	NULL		promotes	NULL				S phase	NULL	entry into			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_16_15836_s_20	15691830	A dual connection links Id2 and pRb: when overexpressed, Id2 overrides the tumor suppressor function of RB, allowing binding of E2F to its target genes, promoting entry into S phase and cell proliferation ( ).	bind
43318	6	10137	7	10	NULL	0	NULL	statement 4			promotes					cell		proliferation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_16_15836_s_20	15691830	A dual connection links Id2 and pRb: when overexpressed, Id2 overrides the tumor suppressor function of RB, allowing binding of E2F to its target genes, promoting entry into S phase and cell proliferation ( ).	bind
35797	1	10139	6	11	NULL	NULL	NULL	Dyn2 dimer	GP		bind			PRD		SNX9	GP		SH3		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_41_42694_s_241	15299020	A Dyn2 dimer is bound  to SNX9 through a PRD-SH3 interaction.	bind
43319	1	10139	7	NULL	NULL	0	NULL	Dyn2 dimer	NULL		bind	NULL		PRD		SNX9	NULL		SH3		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_41_42694_s_241	15299020	A Dyn2 dimer is bound  to SNX9 through a PRD-SH3 interaction.	bind
35799	1	10140	6	11	NULL	NULL	NULL	bilirubin	Chemical		bind					serum albumin	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_73_s_170	7814422	A Dynamic Model for Bilirubin Binding to Human Serum Albumin.	bind
43320	1	10140	7	NULL	NULL	0	NULL	Bilirubin	NULL		bind	NULL				Serum Albumin	NULL	human			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_73_s_170	7814422	A Dynamic Model for Bilirubin Binding to Human Serum Albumin.	bind
35800	1	10141	6	11	NULL	NULL	NULL	dyn	GP	mutant	bind		reduced affinity	K44A		GTP	Chemical				NULL	podosomes in BHK-RSV cells	NULL	NULL	NULL	NULL	gw70_molbiolcell_16_7_3301_s_27	15872089	A dynamin mutant (dynK44A), which binds GTP with reduced affinity (Damke  et al., 1994 ; Warnock  et al., 1995 ), affected actin stress fiber formation and cell shape (Damke  et al., 1994 ) and delayed actin turnover at podosomes in BHK-RSV cells (Ochoa  et al., 2000 ).	bind
35801	2	10141	6	11	NULL	NULL	NULL	statement 1	Process		affects					actin stress fiber	GP	formation of			NULL	podosomes in BHK-RSV cells	NULL	NULL	NULL	NULL	gw70_molbiolcell_16_7_3301_s_27	15872089	A dynamin mutant (dynK44A), which binds GTP with reduced affinity (Damke  et al., 1994 ; Warnock  et al., 1995 ), affected actin stress fiber formation and cell shape (Damke  et al., 1994 ) and delayed actin turnover at podosomes in BHK-RSV cells (Ochoa  et al., 2000 ).	bind
35802	3	10141	6	11	NULL	NULL	NULL	statement 1	Process		affects					cell shape	Cell				NULL	podosomes in BHK-RSV cells	NULL	NULL	NULL	NULL	gw70_molbiolcell_16_7_3301_s_27	15872089	A dynamin mutant (dynK44A), which binds GTP with reduced affinity (Damke  et al., 1994 ; Warnock  et al., 1995 ), affected actin stress fiber formation and cell shape (Damke  et al., 1994 ) and delayed actin turnover at podosomes in BHK-RSV cells (Ochoa  et al., 2000 ).	bind
35803	4	10141	6	11	NULL	NULL	NULL	statement 1	Process		delays					actin turnover	GP				NULL	podosomes in BHK-RSV cells	NULL	NULL	NULL	NULL	gw70_molbiolcell_16_7_3301_s_27	15872089	A dynamin mutant (dynK44A), which binds GTP with reduced affinity (Damke  et al., 1994 ; Warnock  et al., 1995 ), affected actin stress fiber formation and cell shape (Damke  et al., 1994 ) and delayed actin turnover at podosomes in BHK-RSV cells (Ochoa  et al., 2000 ).	bind
43321	1	10141	7	10	NULL	0	NULL	dyn		mutant	binds		reduced affinity	K44A		GTP					NULL	podosomes in BHK-RSV cells	NULL	NULL	NULL	NULL	gw70_molbiolcell_16_7_3301_s_27	15872089	A dynamin mutant (dynK44A), which binds GTP with reduced affinity (Damke  et al., 1994 ; Warnock  et al., 1995 ), affected actin stress fiber formation and cell shape (Damke  et al., 1994 ) and delayed actin turnover at podosomes in BHK-RSV cells (Ochoa  et al., 2000 ).	bind
43322	2	10141	7	10	NULL	0	NULL	statement 1			affects					actin stress fiber		formation of			NULL	podosomes in BHK-RSV cells	NULL	NULL	NULL	NULL	gw70_molbiolcell_16_7_3301_s_27	15872089	A dynamin mutant (dynK44A), which binds GTP with reduced affinity (Damke  et al., 1994 ; Warnock  et al., 1995 ), affected actin stress fiber formation and cell shape (Damke  et al., 1994 ) and delayed actin turnover at podosomes in BHK-RSV cells (Ochoa  et al., 2000 ).	bind
43323	3	10141	7	10	NULL	0	NULL	statement 1			affects					cell shape					NULL	podosomes in BHK-RSV cells	NULL	NULL	NULL	NULL	gw70_molbiolcell_16_7_3301_s_27	15872089	A dynamin mutant (dynK44A), which binds GTP with reduced affinity (Damke  et al., 1994 ; Warnock  et al., 1995 ), affected actin stress fiber formation and cell shape (Damke  et al., 1994 ) and delayed actin turnover at podosomes in BHK-RSV cells (Ochoa  et al., 2000 ).	bind
43324	4	10141	7	10	NULL	0	NULL	statement 1			delays					actin turnover					NULL	podosomes in BHK-RSV cells	NULL	NULL	NULL	NULL	gw70_molbiolcell_16_7_3301_s_27	15872089	A dynamin mutant (dynK44A), which binds GTP with reduced affinity (Damke  et al., 1994 ; Warnock  et al., 1995 ), affected actin stress fiber formation and cell shape (Damke  et al., 1994 ) and delayed actin turnover at podosomes in BHK-RSV cells (Ochoa  et al., 2000 ).	bind
43325	5	10141	7	NULL	NULL	0	NULL	dynK44A	NULL		is	NULL				dynamin mutant	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_7_3301_s_27	15872089	A dynamin mutant (dynK44A), which binds GTP with reduced affinity (Damke  et al., 1994 ; Warnock  et al., 1995 ), affected actin stress fiber formation and cell shape (Damke  et al., 1994 ) and delayed actin turnover at podosomes in BHK-RSV cells (Ochoa  et al., 2000 ).	bind
35804	1	10143	6	11	NULL	NULL	NULL	nuclear protein of 130 kDa	GP	eukaryotic	bind							bacterial		cAMP responsive element	NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochim-biophys-acta_1089_2_1647212_s_1	1647212	A eukaryotic nuclear protein of 130 kDa binds to a bacterial cAMP responsive element..	bind
43328	1	10143	7	10	NULL	0	NULL	nuclear protein of 130 kDa	NULL	eukaryotic	binds to	NULL					NULL	bacterial		cAMP responsive element	NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochim-biophys-acta_1089_2_1647212_s_1	1647212	A eukaryotic nuclear protein of 130 kDa binds to a bacterial cAMP responsive element..	bind
35805	1	10144	6	11	NULL	NULL	NULL	eRF-1	GP		bind					PP2A	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_73_1_68_s_290	10581399	A eukaryotic translational release factor (eRF-1) binds to PP2A and localizes the phosphatase to ribosomes  [ 2.	bind
35806	2	10144	6	11	NULL	NULL	NULL	eRF-1	GP		is					eukaryotic translational release factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_73_1_68_s_290	10581399	A eukaryotic translational release factor (eRF-1) binds to PP2A and localizes the phosphatase to ribosomes  [ 2.	bind
35807	3	10144	6	11	NULL	NULL	NULL	phosphatase	GP		is localized to					ribosomes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_73_1_68_s_290	10581399	A eukaryotic translational release factor (eRF-1) binds to PP2A and localizes the phosphatase to ribosomes  [ 2.	bind
35808	4	10144	6	11	NULL	NULL	NULL	statement 1	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_brainresmolbrainres_73_1_68_s_290	10581399	A eukaryotic translational release factor (eRF-1) binds to PP2A and localizes the phosphatase to ribosomes  [ 2.	bind
43329	1	10144	7	NULL	NULL	0	NULL	eRF-1	NULL		binds to	NULL				PP2A	NULL				NULL		0	NULL	NULL	NULL	gw60_brainresmolbrainres_73_1_68_s_290	10581399	A eukaryotic translational release factor (eRF-1) binds to PP2A and localizes the phosphatase to ribosomes  [ 2.	bind
43330	2	10144	7	NULL	NULL	0	NULL	phosphatases	NULL		localize to	NULL				ribosomes	NULL				NULL		0	NULL	NULL	NULL	gw60_brainresmolbrainres_73_1_68_s_290	10581399	A eukaryotic translational release factor (eRF-1) binds to PP2A and localizes the phosphatase to ribosomes  [ 2.	bind
43331	3	10144	7	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_brainresmolbrainres_73_1_68_s_290	10581399	A eukaryotic translational release factor (eRF-1) binds to PP2A and localizes the phosphatase to ribosomes  [ 2.	bind
43332	4	10144	7	NULL	NULL	0	NULL	eRF-1	NULL		is	NULL				eukaryotic translational release factor	NULL				NULL		0	NULL	NULL	NULL	gw60_brainresmolbrainres_73_1_68_s_290	10581399	A eukaryotic translational release factor (eRF-1) binds to PP2A and localizes the phosphatase to ribosomes  [ 2.	bind
35809	1	10145	6	11	NULL	NULL	NULL	Lipoprotein(a)	Chemical		bind					platelets	CellComponent	human			NULL		NULL	NULL	NULL	NULL	gw60_atherosclerosis_140_1_155_s_161	9733226	A Ezratty, DI Simon and J Loscalzo, Lipoprotein(a) binds to human platelets and attenuates plasminogen binding and activation.	bind
35810	2	10145	6	11	NULL	NULL	NULL	statement 1	Process		attenuates					plasminogen	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_atherosclerosis_140_1_155_s_161	9733226	A Ezratty, DI Simon and J Loscalzo, Lipoprotein(a) binds to human platelets and attenuates plasminogen binding and activation.	bind
35811	3	10145	6	11	NULL	NULL	NULL	statement 1	Process		attenuates					plasminogen	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_atherosclerosis_140_1_155_s_161	9733226	A Ezratty, DI Simon and J Loscalzo, Lipoprotein(a) binds to human platelets and attenuates plasminogen binding and activation.	bind
43333	1	10145	7	NULL	NULL	0	NULL	Lipoprotein	NULL		binds to	NULL				platelets	NULL	human			NULL		0	NULL	NULL	NULL	gw60_atherosclerosis_140_1_155_s_161	9733226	A Ezratty, DI Simon and J Loscalzo, Lipoprotein(a) binds to human platelets and attenuates plasminogen binding and activation.	bind
43334	2	10145	7	NULL	NULL	0	NULL	statement 1	NULL		attenuates	NULL				plasminogen	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_atherosclerosis_140_1_155_s_161	9733226	A Ezratty, DI Simon and J Loscalzo, Lipoprotein(a) binds to human platelets and attenuates plasminogen binding and activation.	bind
43335	3	10145	7	NULL	NULL	0	NULL	statement 1	NULL		attenuates	NULL				plasminogen	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_atherosclerosis_140_1_155_s_161	9733226	A Ezratty, DI Simon and J Loscalzo, Lipoprotein(a) binds to human platelets and attenuates plasminogen binding and activation.	bind
35812	1	10147	6	11	NULL	NULL	NULL	NIF	GP	125I-labeled	bind							recombinant	I-domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_21_18769_s_109	11880366	A facile binding assay for quantifying NIF binding to the recombinant I-domains was developed by measuring the binding of 125I-NIF to the recombinant I-domains captured onto glutathione-Sepharose.	bind
44004	1	10147	7	10	NULL	0	NULL	NIF	NULL	125I-labeled	bind	NULL					NULL	recombinant	I-domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_21_18769_s_109	11880366	A facile binding assay for quantifying NIF binding to the recombinant I-domains was developed by measuring the binding of 125I-NIF to the recombinant I-domains captured onto glutathione-Sepharose.	bind
35813	1	10148	6	11	NULL	NULL	NULL	DSC	ResearchActivity		bind		specifically							MCB cis-element	NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_6_1577_s_11	9614195	A factor complex that specifically binds to the MCB  cis-element was initially identified in budding yeast by gel shift assay and called DSC (Lowndes  et al., 1991  ).	bind
35814	2	10148	6	11	NULL	NULL	NULL	DSC	ResearchActivity		is identified in					budding yeast	Organism				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_6_1577_s_11	9614195	A factor complex that specifically binds to the MCB  cis-element was initially identified in budding yeast by gel shift assay and called DSC (Lowndes  et al., 1991  ).	bind
44005	1	10148	7	10	NULL	0	NULL	DSC	NULL		bind	NULL	specifically				NULL			MCB cis-element	NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_6_1577_s_11	9614195	A factor complex that specifically binds to the MCB  cis-element was initially identified in budding yeast by gel shift assay and called DSC (Lowndes  et al., 1991  ).	bind
49602	2	10148	7	10	NULL	0	NULL	DSC	NULL		is identified in	NULL				budding yeast	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_9_6_1577_s_11	9614195	A factor complex that specifically binds to the MCB  cis-element was initially identified in budding yeast by gel shift assay and called DSC (Lowndes  et al., 1991  ).	bind
35816	1	10150	6	11	NULL	NULL	NULL	factor VIII	GP		bind					von Willebrand factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_nature_402_6760_439_s_174	10586887	A factor VIII neutralizing monoclonal antibody and a human inhibitor alloantibody recognizing epitopes in the C2 domain inhibit factor VIII binding to von Willebrand factor and to phosphatidylserine.	bind
35817	2	10150	6	11	NULL	NULL	NULL	factor VIII neutralizing monoclonal antibody	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_nature_402_6760_439_s_174	10586887	A factor VIII neutralizing monoclonal antibody and a human inhibitor alloantibody recognizing epitopes in the C2 domain inhibit factor VIII binding to von Willebrand factor and to phosphatidylserine.	bind
35818	3	10150	6	11	NULL	NULL	NULL	factor VIII	GP		bind					phosphatidylserine	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_nature_402_6760_439_s_174	10586887	A factor VIII neutralizing monoclonal antibody and a human inhibitor alloantibody recognizing epitopes in the C2 domain inhibit factor VIII binding to von Willebrand factor and to phosphatidylserine.	bind
35819	4	10150	6	11	NULL	NULL	NULL	factor VIII neutralizing monoclonal antibody	GP		inhibits					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_nature_402_6760_439_s_174	10586887	A factor VIII neutralizing monoclonal antibody and a human inhibitor alloantibody recognizing epitopes in the C2 domain inhibit factor VIII binding to von Willebrand factor and to phosphatidylserine.	bind
35820	5	10150	6	11	NULL	NULL	NULL	inhibitor alloantibody	GP	human	recognize							epitopes in	C2 domain		NULL		NULL	NULL	NULL	NULL	gw60_nature_402_6760_439_s_174	10586887	A factor VIII neutralizing monoclonal antibody and a human inhibitor alloantibody recognizing epitopes in the C2 domain inhibit factor VIII binding to von Willebrand factor and to phosphatidylserine.	bind
35821	6	10150	6	11	NULL	NULL	NULL	statement 5	Process		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_nature_402_6760_439_s_174	10586887	A factor VIII neutralizing monoclonal antibody and a human inhibitor alloantibody recognizing epitopes in the C2 domain inhibit factor VIII binding to von Willebrand factor and to phosphatidylserine.	bind
35822	7	10150	6	11	NULL	NULL	NULL	statement 5	Process		inhibits					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_nature_402_6760_439_s_174	10586887	A factor VIII neutralizing monoclonal antibody and a human inhibitor alloantibody recognizing epitopes in the C2 domain inhibit factor VIII binding to von Willebrand factor and to phosphatidylserine.	bind
44010	1	10150	7	NULL	NULL	0	NULL	factor VIII	NULL		bind	NULL				von Willebrand factor 	NULL				NULL		0	NULL	NULL	NULL	gw60_nature_402_6760_439_s_174	10586887	A factor VIII neutralizing monoclonal antibody and a human inhibitor alloantibody recognizing epitopes in the C2 domain inhibit factor VIII binding to von Willebrand factor and to phosphatidylserine.	bind
44012	2	10150	7	NULL	NULL	0	NULL	factor VIII	NULL		bind	NULL				phosphatidylserine	NULL				NULL		0	NULL	NULL	NULL	gw60_nature_402_6760_439_s_174	10586887	A factor VIII neutralizing monoclonal antibody and a human inhibitor alloantibody recognizing epitopes in the C2 domain inhibit factor VIII binding to von Willebrand factor and to phosphatidylserine.	bind
44018	3	10150	7	NULL	NULL	0	NULL	inhibitor alloantibody	NULL	human	recognize	NULL					NULL	epitopes in	 C2 domain		NULL		NULL	NULL	NULL	NULL	gw60_nature_402_6760_439_s_174	10586887	A factor VIII neutralizing monoclonal antibody and a human inhibitor alloantibody recognizing epitopes in the C2 domain inhibit factor VIII binding to von Willebrand factor and to phosphatidylserine.	bind
44020	4	10150	7	NULL	NULL	0	NULL	statement 3	NULL		inhibit	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nature_402_6760_439_s_174	10586887	A factor VIII neutralizing monoclonal antibody and a human inhibitor alloantibody recognizing epitopes in the C2 domain inhibit factor VIII binding to von Willebrand factor and to phosphatidylserine.	bind
44021	5	10150	7	NULL	NULL	0	NULL	statement 3	NULL		inhibit	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nature_402_6760_439_s_174	10586887	A factor VIII neutralizing monoclonal antibody and a human inhibitor alloantibody recognizing epitopes in the C2 domain inhibit factor VIII binding to von Willebrand factor and to phosphatidylserine.	bind
44023	7	10150	7	NULL	NULL	0	NULL	factor VIII neutralizing monoclonal antibody	NULL		inhibit	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nature_402_6760_439_s_174	10586887	A factor VIII neutralizing monoclonal antibody and a human inhibitor alloantibody recognizing epitopes in the C2 domain inhibit factor VIII binding to von Willebrand factor and to phosphatidylserine.	bind
50242	6	10150	7	NULL	NULL	0	NULL	factor VIII neutralizing monoclonal antibody	NULL		inhibit	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nature_402_6760_439_s_174	10586887	A factor VIII neutralizing monoclonal antibody and a human inhibitor alloantibody recognizing epitopes in the C2 domain inhibit factor VIII binding to von Willebrand factor and to phosphatidylserine.	bind
35823	1	10151	6	11	NULL	NULL	NULL	U2AF	GP		is required for					U2 snRNP	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_7_1010_s_534	9531538	A factor, U2AF, is required for U2 snRNP binding and splicing complex assembly.	bind
35824	2	10151	6	11	NULL	NULL	NULL	U2AF	GP		is required for					splicing complex	GP	assembly of			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_7_1010_s_534	9531538	A factor, U2AF, is required for U2 snRNP binding and splicing complex assembly.	bind
44024	1	10151	7	NULL	NULL	0	NULL	U2AF factor	NULL		is required for	NULL				U2 snRNP	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_genesdev_12_7_1010_s_534	9531538	A factor, U2AF, is required for U2 snRNP binding and splicing complex assembly.	bind
44025	2	10151	7	NULL	NULL	0	NULL	U2AF  factor	NULL		is required for	NULL				splicing complex	NULL	assembly of			NULL		0	NULL	NULL	NULL	gw60_genesdev_12_7_1010_s_534	9531538	A factor, U2AF, is required for U2 snRNP binding and splicing complex assembly.	bind
35825	1	10152	6	11	NULL	NULL	NULL	Xa7	GP	Xanthomonas oryzae pv. oryzae	bind					DNA	NucleicAcid			AT-rich 	NULL		NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_60_0_425_s_224	16753033	A family  member from  Xanthomonas oryzae pv.  oryzae, Xa7, binds AT-rich DNA ( 134), but specific host DNA binding sites have not been identified.	bind
44026	1	10152	7	10	NULL	0	NULL	Xa7	NULL	Xanthomonas oryzae pv. oryzae	binds	NULL				DNA	NULL			AT-rich	NULL		NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_60_0_425_s_224	16753033	A family  member from  Xanthomonas oryzae pv.  oryzae, Xa7, binds AT-rich DNA ( 134), but specific host DNA binding sites have not been identified.	bind
35826	1	10154	6	11	NULL	NULL	NULL	MBD	GP		is a					methyl-CpG-binding domain	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_2_397_s_22	16415179	A family of DNA binding proteins harboring a methyl-CpG-binding domain (MBD) recognizes and binds to methylated CpG sequences ( ).	bind
35827	2	10154	6	11	NULL	NULL	NULL	DNA-binding protein	GP		bind			MBD				methylated		CpG sequences	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_2_397_s_22	16415179	A family of DNA binding proteins harboring a methyl-CpG-binding domain (MBD) recognizes and binds to methylated CpG sequences ( ).	bind
35828	3	10154	6	11	NULL	NULL	NULL	DNA-binding protein	GP		recognizes			MBD				methylated		CpG sequences	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_2_397_s_22	16415179	A family of DNA binding proteins harboring a methyl-CpG-binding domain (MBD) recognizes and binds to methylated CpG sequences ( ).	bind
44031	1	10154	7	10	NULL	0	NULL	DNA-binding protein			recognizes			MBD				methylated		CpG sequences	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_2_397_s_22	16415179	A family of DNA binding proteins harboring a methyl-CpG-binding domain (MBD) recognizes and binds to methylated CpG sequences ( ).	bind
44033	2	10154	7	10	NULL	0	NULL	DNA-binding protein			binds			MBD				methylated		CpG sequences	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_2_397_s_22	16415179	A family of DNA binding proteins harboring a methyl-CpG-binding domain (MBD) recognizes and binds to methylated CpG sequences ( ).	bind
44035	3	10154	7	NULL	NULL	0	NULL	MBD	NULL		is	NULL				methyl-CpG-binding domain	NULL				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_34_2_397_s_22	16415179	A family of DNA binding proteins harboring a methyl-CpG-binding domain (MBD) recognizes and binds to methylated CpG sequences ( ).	bind
35829	1	10155	6	11	NULL	NULL	NULL	lymphoid Ig-like receptor	GP	human	bind					MHC class I molecules	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiophysbiomol_32_0_93_s_389	12471063	A family of human  lymphoid and myeloid Ig-like receptors, some of which bind to MHC class I molecules.	bind
35830	2	10155	6	11	NULL	NULL	NULL	myeloid Ig-like receptor	GP	human	bind					MHC class I molecules	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiophysbiomol_32_0_93_s_389	12471063	A family of human  lymphoid and myeloid Ig-like receptors, some of which bind to MHC class I molecules.	bind
44037	1	10155	7	NULL	NULL	0	NULL	lymphoid Ig-like receptors	NULL	human	binds to	NULL				MHC class I  molecules	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevbiophysbiomol_32_0_93_s_389	12471063	A family of human  lymphoid and myeloid Ig-like receptors, some of which bind to MHC class I molecules.	bind
44038	2	10155	7	NULL	NULL	0	NULL	myeloid Ig-like receptors	NULL	human	binds to	NULL				MHC class I  molecules	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevbiophysbiomol_32_0_93_s_389	12471063	A family of human  lymphoid and myeloid Ig-like receptors, some of which bind to MHC class I molecules.	bind
35831	1	10157	6	11	NULL	NULL	NULL	LIM	GP		is a type of					homeodomain protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_development_130_17_4161_s_417	12874135	A family of LIM domain-associated cofactors confer transcriptional synergism between LIM and Otx homeodomain proteins.	bind
35832	2	10157	6	11	NULL	NULL	NULL	Otx	GP		is a type of					homeodomain protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_development_130_17_4161_s_417	12874135	A family of LIM domain-associated cofactors confer transcriptional synergism between LIM and Otx homeodomain proteins.	bind
35833	3	10157	6	11	NULL	NULL	NULL	LIM	GP		synergizes with		transcriptionaly			Otx	GP				NULL		NULL	NULL	NULL	NULL	gw60_development_130_17_4161_s_417	12874135	A family of LIM domain-associated cofactors confer transcriptional synergism between LIM and Otx homeodomain proteins.	bind
35834	4	10157	6	11	NULL	NULL	NULL	LIM domain-associated cofactors	GP		confer					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_development_130_17_4161_s_417	12874135	A family of LIM domain-associated cofactors confer transcriptional synergism between LIM and Otx homeodomain proteins.	bind
44039	1	10157	7	10	NULL	0	NULL	LIM	NULL		synergize with	NULL	transcriptionally			Otx	NULL				NULL		NULL	NULL	NULL	NULL	gw60_development_130_17_4161_s_417	12874135	A family of LIM domain-associated cofactors confer transcriptional synergism between LIM and Otx homeodomain proteins.	bind
44040	2	10157	7	10	NULL	0	NULL	LIM domain-associated cofactors	NULL		confer	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_development_130_17_4161_s_417	12874135	A family of LIM domain-associated cofactors confer transcriptional synergism between LIM and Otx homeodomain proteins.	bind
49662	3	10157	7	10	NULL	0	NULL	LIM	NULL		is a type of	NULL				homeodomain protein	NULL				NULL		0	NULL	NULL	NULL	gw60_development_130_17_4161_s_417	12874135	A family of LIM domain-associated cofactors confer transcriptional synergism between LIM and Otx homeodomain proteins.	bind
49663	4	10157	7	10	NULL	0	NULL	Otx	NULL		is a type of	NULL				homeodomain protein	NULL				NULL		0	NULL	NULL	NULL	gw60_development_130_17_4161_s_417	12874135	A family of LIM domain-associated cofactors confer transcriptional synergism between LIM and Otx homeodomain proteins.	bind
35835	1	10159	6	11	NULL	NULL	NULL	Na+/H+ exchanger regulatory factor	GP		bind								C terminus (D(SST)- X-L)		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_6_3729_s_139	10660517	A family of PDZ-binding domain proteins, including the Na+/H+ exchanger regulatory factor ( 65) and ezrin-binding protein 50 ( 66), bind to the C terminus (D(SST)- X-L) (Fig.  2).	bind
35836	2	10159	6	11	NULL	NULL	NULL	ezrin-binding protein 50	GP		bind								C terminus (D(SST)- X-L)		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_6_3729_s_139	10660517	A family of PDZ-binding domain proteins, including the Na+/H+ exchanger regulatory factor ( 65) and ezrin-binding protein 50 ( 66), bind to the C terminus (D(SST)- X-L) (Fig.  2).	bind
35837	3	10159	6	11	NULL	NULL	NULL	Na+/H+ exchanger regulatory factor	GP		is a type of					PDZ-binding domain protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_6_3729_s_139	10660517	A family of PDZ-binding domain proteins, including the Na+/H+ exchanger regulatory factor ( 65) and ezrin-binding protein 50 ( 66), bind to the C terminus (D(SST)- X-L) (Fig.  2).	bind
35838	4	10159	6	11	NULL	NULL	NULL	ezrin-binding protein 50	GP		is a type of					PDZ-binding domain protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_6_3729_s_139	10660517	A family of PDZ-binding domain proteins, including the Na+/H+ exchanger regulatory factor ( 65) and ezrin-binding protein 50 ( 66), bind to the C terminus (D(SST)- X-L) (Fig.  2).	bind
44042	1	10159	7	NULL	NULL	0	NULL	Na+/H+ exchanger regulatory factor	NULL		bind	NULL					NULL		C terminus  (D(SST)- X-L)		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_6_3729_s_139	10660517	A family of PDZ-binding domain proteins, including the Na+/H+ exchanger regulatory factor ( 65) and ezrin-binding protein 50 ( 66), bind to the C terminus (D(SST)- X-L) (Fig.  2).	bind
44043	2	10159	7	NULL	NULL	0	NULL	ezrin-binding protein	NULL		bind	NULL					NULL		C terminus  (D(SST)- X-L)		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_6_3729_s_139	10660517	A family of PDZ-binding domain proteins, including the Na+/H+ exchanger regulatory factor ( 65) and ezrin-binding protein 50 ( 66), bind to the C terminus (D(SST)- X-L) (Fig.  2).	bind
44044	3	10159	7	NULL	NULL	0	NULL	Na+/H+ exchanger regulatory factor	NULL		is a type of	NULL				PDZ-binding domain proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_6_3729_s_139	10660517	A family of PDZ-binding domain proteins, including the Na+/H+ exchanger regulatory factor ( 65) and ezrin-binding protein 50 ( 66), bind to the C terminus (D(SST)- X-L) (Fig.  2).	bind
44045	4	10159	7	NULL	NULL	0	NULL	ezrin-binding protein	NULL		is a type of	NULL				PDZ-binding domain proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_6_3729_s_139	10660517	A family of PDZ-binding domain proteins, including the Na+/H+ exchanger regulatory factor ( 65) and ezrin-binding protein 50 ( 66), bind to the C terminus (D(SST)- X-L) (Fig.  2).	bind
35839	1	10160	6	11	NULL	NULL	NULL	von Hippel-Lindau tumor suppressor protein	GP		bind					HIF-1alpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_26_23111_s_20	11943784	A family of prolyl hydroxylase enzymes regulates the binding of von Hippel-Lindau tumor suppressor protein to HIF-1alpha by hydroxylating key proline residues on the HIF-1alpha protein ( 17-20).	bind
35840	2	10160	6	11	NULL	NULL	NULL	family of prolyl hydroxylase enzymes	GP		regulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_26_23111_s_20	11943784	A family of prolyl hydroxylase enzymes regulates the binding of von Hippel-Lindau tumor suppressor protein to HIF-1alpha by hydroxylating key proline residues on the HIF-1alpha protein ( 17-20).	bind
35841	3	10160	6	11	NULL	NULL	NULL	family of prolyl hydroxylase enzymes	GP		hydroxylate					HIF-1alpha protein	GP		proline residues		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_26_23111_s_20	11943784	A family of prolyl hydroxylase enzymes regulates the binding of von Hippel-Lindau tumor suppressor protein to HIF-1alpha by hydroxylating key proline residues on the HIF-1alpha protein ( 17-20).	bind
35842	4	10160	6	11	NULL	NULL	NULL	statement 2	Process		occurs by					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_26_23111_s_20	11943784	A family of prolyl hydroxylase enzymes regulates the binding of von Hippel-Lindau tumor suppressor protein to HIF-1alpha by hydroxylating key proline residues on the HIF-1alpha protein ( 17-20).	bind
44046	1	10160	7	NULL	NULL	0	NULL	von Hippel-Lindau tumor suppressor protein	NULL		bind	NULL				HIF-1alpha	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23111_s_20	11943784	A family of prolyl hydroxylase enzymes regulates the binding of von Hippel-Lindau tumor suppressor protein to HIF-1alpha by hydroxylating key proline residues on the HIF-1alpha protein ( 17-20).	bind
44047	2	10160	7	NULL	NULL	0	NULL	statement 1	NULL		occurs upon	NULL				HIF-1alpha protein	NULL	hydroxylation of	key proline residues		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23111_s_20	11943784	A family of prolyl hydroxylase enzymes regulates the binding of von Hippel-Lindau tumor suppressor protein to HIF-1alpha by hydroxylating key proline residues on the HIF-1alpha protein ( 17-20).	bind
44048	3	10160	7	NULL	NULL	0	NULL	prolyl hydroxylase enzymes	NULL		regulate	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23111_s_20	11943784	A family of prolyl hydroxylase enzymes regulates the binding of von Hippel-Lindau tumor suppressor protein to HIF-1alpha by hydroxylating key proline residues on the HIF-1alpha protein ( 17-20).	bind
35843	1	10161	6	11	NULL	NULL	NULL	IGFBPs	GP		bind					IGF-I	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_endocrinology_138_11_9348216_s_2	9348216	A family of six insulin-like growth factor binding proteins (IGFBPs) bind  IGF-I and modulate its biological activity.	bind
35844	2	10161	6	11	NULL	NULL	NULL	statement 1	GP		modulates					IGF-I	GP	biological activity of			NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_endocrinology_138_11_9348216_s_2	9348216	A family of six insulin-like growth factor binding proteins (IGFBPs) bind  IGF-I and modulate its biological activity.	bind
35845	3	10161	6	11	NULL	NULL	NULL	IGFBP	GP		is					insulin-like growth factor binding protein	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_endocrinology_138_11_9348216_s_2	9348216	A family of six insulin-like growth factor binding proteins (IGFBPs) bind  IGF-I and modulate its biological activity.	bind
44049	1	10161	7	NULL	NULL	0	NULL	IGFBPs	NULL		bind	NULL				IGF-I	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_endocrinology_138_11_9348216_s_2	9348216	A family of six insulin-like growth factor binding proteins (IGFBPs) bind  IGF-I and modulate its biological activity.	bind
44050	2	10161	7	NULL	NULL	0	NULL	statement 1	NULL		modulate	NULL				IGF-I	NULL	biological activity of			NULL		0	NULL	NULL	NULL	abs-batch0620-0649_endocrinology_138_11_9348216_s_2	9348216	A family of six insulin-like growth factor binding proteins (IGFBPs) bind  IGF-I and modulate its biological activity.	bind
44051	3	10161	7	NULL	NULL	0	NULL	IGFBPs	NULL		is	NULL				insulin-like growth factor binding proteins	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_endocrinology_138_11_9348216_s_2	9348216	A family of six insulin-like growth factor binding proteins (IGFBPs) bind  IGF-I and modulate its biological activity.	bind
35846	1	10162	6	11	NULL	NULL	NULL	AKAP	GP		is a type of					anchoring protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_512_1_91_s_8	11852058	A family of these anchoring proteins (AKAP) bind both cAMP-dependent PK (PKA) and PPs targeting them to specific cellular membranes [ 7,   8 and   9].	bind
35847	2	10162	6	11	NULL	NULL	NULL	AKAP	GP		bind					PKA	GP	cAMP-dependent			NULL		NULL	NULL	NULL	NULL	gw60_febslett_512_1_91_s_8	11852058	A family of these anchoring proteins (AKAP) bind both cAMP-dependent PK (PKA) and PPs targeting them to specific cellular membranes [ 7,   8 and   9].	bind
35848	3	10162	6	11	NULL	NULL	NULL	AKAP	GP		bind					PP	GP	cAMP-dependent			NULL		NULL	NULL	NULL	NULL	gw60_febslett_512_1_91_s_8	11852058	A family of these anchoring proteins (AKAP) bind both cAMP-dependent PK (PKA) and PPs targeting them to specific cellular membranes [ 7,   8 and   9].	bind
44052	1	10162	7	NULL	NULL	0	NULL	AKAP	NULL		bind	NULL				PKA	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_512_1_91_s_8	11852058	A family of these anchoring proteins (AKAP) bind both cAMP-dependent PK (PKA) and PPs targeting them to specific cellular membranes [ 7,   8 and   9].	bind
44053	2	10162	7	NULL	NULL	0	NULL	AKAP	NULL		bind	NULL				PPs	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_512_1_91_s_8	11852058	A family of these anchoring proteins (AKAP) bind both cAMP-dependent PK (PKA) and PPs targeting them to specific cellular membranes [ 7,   8 and   9].	bind
44054	3	10162	7	11	NULL	NULL	NULL	PKA	GP		targeted to					cellular membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_febslett_512_1_91_s_8	11852058	A family of these anchoring proteins (AKAP) bind both cAMP-dependent PK (PKA) and PPs targeting them to specific cellular membranes [ 7,   8 and   9].	bind
44055	4	10162	7	11	NULL	NULL	NULL	PPs	GP		targeted to					cellular membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_febslett_512_1_91_s_8	11852058	A family of these anchoring proteins (AKAP) bind both cAMP-dependent PK (PKA) and PPs targeting them to specific cellular membranes [ 7,   8 and   9].	bind
44056	5	10162	7	11	NULL	NULL	NULL	statement 1	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_512_1_91_s_8	11852058	A family of these anchoring proteins (AKAP) bind both cAMP-dependent PK (PKA) and PPs targeting them to specific cellular membranes [ 7,   8 and   9].	bind
44057	6	10162	7	11	NULL	NULL	NULL	statement 2	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_512_1_91_s_8	11852058	A family of these anchoring proteins (AKAP) bind both cAMP-dependent PK (PKA) and PPs targeting them to specific cellular membranes [ 7,   8 and   9].	bind
44058	7	10162	7	NULL	NULL	0	NULL	AKAP	NULL		is a type of	NULL				anchoring proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_512_1_91_s_8	11852058	A family of these anchoring proteins (AKAP) bind both cAMP-dependent PK (PKA) and PPs targeting them to specific cellular membranes [ 7,   8 and   9].	bind
44059	8	10162	7	11	NULL	NULL	NULL	PKA	GP		is					cAMP-dependent PK	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_512_1_91_s_8	11852058	A family of these anchoring proteins (AKAP) bind both cAMP-dependent PK (PKA) and PPs targeting them to specific cellular membranes [ 7,   8 and   9].	bind
35849	1	10163	6	NULL	NULL	0	NULL	family of ubiquitin-like proteins	NULL		bind	NULL				Hsp70-like Stch	NULL		ATPase domain		NULL		0	NULL	NULL	NULL	abs-batch0720-0739_febs-lett_467_2-3_10675567_s_1	10675567	A family of ubiquitin-like proteins binds the ATPase domain of Hsp70-like Stch..	bind
44060	1	10163	7	NULL	NULL	0	NULL	ubiquitin-like proteins	NULL		binds	NULL				Hsp70-like Stch	NULL		ATPase domain		NULL		0	NULL	NULL	NULL	abs-batch0720-0739_febs-lett_467_2-3_10675567_s_1	10675567	A family of ubiquitin-like proteins binds the ATPase domain of Hsp70-like Stch..	bind
35850	1	10165	6	11	NULL	NULL	NULL	Crk	GP		bind					focal adhesion proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_43_35953_s_168	16123042	A far Western analysis was used to determine whether disruption of the interaction by ADP-ribosylation with focal adhesion proteins could be attributed to direct inhibition of Crk binding to the focal adhesion proteins.	bind
44061	1	10165	7	NULL	NULL	0	NULL	Crk	NULL		bind	NULL				focal adhesion proteins	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_43_35953_s_168	16123042	A far Western analysis was used to determine whether disruption of the interaction by ADP-ribosylation with focal adhesion proteins could be attributed to direct inhibition of Crk binding to the focal adhesion proteins.	bind
35851	1	10167	6	11	NULL	NULL	NULL	virus	Organism		bind					host cell membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_68_0_863_s_88	10872468	A fascinating aspect of viral infection   is that in most cases, binding of the virus to the host cell membrane and fusion   of the viral membrane with this membrane are carried out by a single protein   referred to as the viral fusion protein.	bind
35853	2	10167	6	11	NULL	NULL	NULL	viral fusion protein	GP		carries out					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_68_0_863_s_88	10872468	A fascinating aspect of viral infection   is that in most cases, binding of the virus to the host cell membrane and fusion   of the viral membrane with this membrane are carried out by a single protein   referred to as the viral fusion protein.	bind
35855	3	10167	6	11	NULL	NULL	NULL	viral cell membrane	CellComponent		fused with					host cell membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_68_0_863_s_88	10872468	A fascinating aspect of viral infection   is that in most cases, binding of the virus to the host cell membrane and fusion   of the viral membrane with this membrane are carried out by a single protein   referred to as the viral fusion protein.	bind
35856	4	10167	6	11	NULL	NULL	NULL	viral fusion protein	GP		carries out					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_68_0_863_s_88	10872468	A fascinating aspect of viral infection   is that in most cases, binding of the virus to the host cell membrane and fusion   of the viral membrane with this membrane are carried out by a single protein   referred to as the viral fusion protein.	bind
44076	1	10167	7	NULL	NULL	0	NULL	virus	NULL		bind	NULL				host cell membrane	NULL				NULL		0	NULL	NULL	NULL	gw60_annrevbiochem_68_0_863_s_88	10872468	A fascinating aspect of viral infection   is that in most cases, binding of the virus to the host cell membrane and fusion   of the viral membrane with this membrane are carried out by a single protein   referred to as the viral fusion protein.	bind
44078	2	10167	7	NULL	NULL	0	NULL	viral membrane	NULL		fuse with	NULL				host cell membrane	NULL				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_68_0_863_s_88	10872468	A fascinating aspect of viral infection   is that in most cases, binding of the virus to the host cell membrane and fusion   of the viral membrane with this membrane are carried out by a single protein   referred to as the viral fusion protein.	bind
44081	3	10167	7	NULL	NULL	0	NULL	viral fusion protein	NULL		carries out	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_annrevbiochem_68_0_863_s_88	10872468	A fascinating aspect of viral infection   is that in most cases, binding of the virus to the host cell membrane and fusion   of the viral membrane with this membrane are carried out by a single protein   referred to as the viral fusion protein.	bind
49664	4	10167	7	10	NULL	0	NULL	viral fusion protein	NULL		carries out	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_annrevbiochem_68_0_863_s_88	10872468	A fascinating aspect of viral infection   is that in most cases, binding of the virus to the host cell membrane and fusion   of the viral membrane with this membrane are carried out by a single protein   referred to as the viral fusion protein.	bind
35857	1	10169	6	11	NULL	NULL	NULL	BASI	GP		bind					AMY2	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1696_2_145_s_201	14871655	A fast and tight simple two-step mechanism was determined for the binding of BASI  to AMY2 [ 85].	bind
44085	1	10169	7	NULL	NULL	0	NULL	BASI	NULL		bind	NULL				AMY2	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1696_2_145_s_201	14871655	A fast and tight simple two-step mechanism was determined for the binding of BASI  to AMY2 [ 85].	bind
35859	1	10170	6	11	NULL	NULL	NULL	Pi	Chemical		bind					mIPS	GP	recombinant			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_12_11475_s_107	15653679	A fast exchange analysis (deltanuobs - deltanuo = ( Eodeltab)/( KD +  Lo), where (deltanuobs - deltanuo) was the difference in line width for free Pi at a given concentration and Pi when enzyme was present,  Eo was the total enzyme concentration, and  Lo was the total Pi concentration) was used to estimate the enzyme bound line width, deltab, and  KD for Pi binding to recombinant mIPS.	bind
44088	1	10170	7	NULL	NULL	0	NULL	Pi	NULL		bind	NULL				mIPS	NULL	recombinant			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_12_11475_s_107	15653679	A fast exchange analysis (deltanuobs - deltanuo = ( Eodeltab)/( KD +  Lo), where (deltanuobs - deltanuo) was the difference in line width for free Pi at a given concentration and Pi when enzyme was present,  Eo was the total enzyme concentration, and  Lo was the total Pi concentration) was used to estimate the enzyme bound line width, deltab, and  KD for Pi binding to recombinant mIPS.	bind
36300	1	10171	6	11	NULL	NULL	NULL	LRDD	AminoAcid		is similar to		significantly	intermediate region		ankyrin	GP		spectrin binding domain		NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1478_2_280_s_114	10825539	A FastA search of the GenBank database using the full-length LRDD (753 aa) revealed that the intermediate region of LRDD shows significant similarity with the spectrin binding domain of ankyrins.	bind
44091	1	10171	7	10	NULL	0	NULL	LRDD	NULL		is similar to	NULL	significantly	intermediate region		ankyrins	NULL		spectrin binding domain		NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1478_2_280_s_114	10825539	A FastA search of the GenBank database using the full-length LRDD (753 aa) revealed that the intermediate region of LRDD shows significant similarity with the spectrin binding domain of ankyrins.	bind
35874	1	10172	6	11	NULL	NULL	NULL	ARF	GP		is					ADP-ribosylation factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_2_281_s_8	15657398	A favored current model for how this coupling is achieved, known as the priming complex model ( ), proposes that the activated (GTP-bound) form of an ADP ribosylation factor (ARF) - like small GTPase promotes the binding of coat proteins onto the cytoplasmic domain of transmembrane cargo proteins to form a key intermediate that drives both cargo sorting and vesicle formation.	bind
35875	2	10172	6	11	NULL	NULL	NULL	GTP	Chemical		bind					ARF	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_2_281_s_8	15657398	A favored current model for how this coupling is achieved, known as the priming complex model ( ), proposes that the activated (GTP-bound) form of an ADP ribosylation factor (ARF) - like small GTPase promotes the binding of coat proteins onto the cytoplasmic domain of transmembrane cargo proteins to form a key intermediate that drives both cargo sorting and vesicle formation.	bind
35877	3	10172	6	11	NULL	NULL	NULL	ARF	GP		is a type of					small GTPase	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_2_281_s_8	15657398	A favored current model for how this coupling is achieved, known as the priming complex model ( ), proposes that the activated (GTP-bound) form of an ADP ribosylation factor (ARF) - like small GTPase promotes the binding of coat proteins onto the cytoplasmic domain of transmembrane cargo proteins to form a key intermediate that drives both cargo sorting and vesicle formation.	bind
35879	4	10172	6	11	NULL	NULL	NULL	coat proteins	GP		bind					transmembrane cargo proteins	GP		cytoplasmic domain		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_2_281_s_8	15657398	A favored current model for how this coupling is achieved, known as the priming complex model ( ), proposes that the activated (GTP-bound) form of an ADP ribosylation factor (ARF) - like small GTPase promotes the binding of coat proteins onto the cytoplasmic domain of transmembrane cargo proteins to form a key intermediate that drives both cargo sorting and vesicle formation.	bind
35881	5	10172	6	11	NULL	NULL	NULL	statement 2	Process		promotes					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_2_281_s_8	15657398	A favored current model for how this coupling is achieved, known as the priming complex model ( ), proposes that the activated (GTP-bound) form of an ADP ribosylation factor (ARF) - like small GTPase promotes the binding of coat proteins onto the cytoplasmic domain of transmembrane cargo proteins to form a key intermediate that drives both cargo sorting and vesicle formation.	bind
35887	6	10172	6	11	NULL	NULL	NULL	statement 4	Process		forms 					intermediate	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_2_281_s_8	15657398	A favored current model for how this coupling is achieved, known as the priming complex model ( ), proposes that the activated (GTP-bound) form of an ADP ribosylation factor (ARF) - like small GTPase promotes the binding of coat proteins onto the cytoplasmic domain of transmembrane cargo proteins to form a key intermediate that drives both cargo sorting and vesicle formation.	bind
35889	7	10172	6	11	NULL	NULL	NULL	statement 6	Process		plays a role in					cargo sorting	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_2_281_s_8	15657398	A favored current model for how this coupling is achieved, known as the priming complex model ( ), proposes that the activated (GTP-bound) form of an ADP ribosylation factor (ARF) - like small GTPase promotes the binding of coat proteins onto the cytoplasmic domain of transmembrane cargo proteins to form a key intermediate that drives both cargo sorting and vesicle formation.	bind
35891	8	10172	6	11	NULL	NULL	NULL	statement 6	Process		plays a role in					vesicle formation	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_2_281_s_8	15657398	A favored current model for how this coupling is achieved, known as the priming complex model ( ), proposes that the activated (GTP-bound) form of an ADP ribosylation factor (ARF) - like small GTPase promotes the binding of coat proteins onto the cytoplasmic domain of transmembrane cargo proteins to form a key intermediate that drives both cargo sorting and vesicle formation.	bind
44096	1	10172	7	NULL	NULL	0	NULL	coat proteins	NULL		bind	NULL				transmembrane cargo proteins	NULL		cytoplasmic domain		NULL		0	NULL	NULL	NULL	gw70_cellbiol_168_2_281_s_8	15657398	A favored current model for how this coupling is achieved, known as the priming complex model ( ), proposes that the activated (GTP-bound) form of an ADP ribosylation factor (ARF) - like small GTPase promotes the binding of coat proteins onto the cytoplasmic domain of transmembrane cargo proteins to form a key intermediate that drives both cargo sorting and vesicle formation.	bind
44098	2	10172	7	NULL	NULL	0	NULL	ARF	NULL	activated	promotes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_168_2_281_s_8	15657398	A favored current model for how this coupling is achieved, known as the priming complex model ( ), proposes that the activated (GTP-bound) form of an ADP ribosylation factor (ARF) - like small GTPase promotes the binding of coat proteins onto the cytoplasmic domain of transmembrane cargo proteins to form a key intermediate that drives both cargo sorting and vesicle formation.	bind
44100	3	10172	7	NULL	NULL	0	NULL	small GTPase	NULL		promotes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_168_2_281_s_8	15657398	A favored current model for how this coupling is achieved, known as the priming complex model ( ), proposes that the activated (GTP-bound) form of an ADP ribosylation factor (ARF) - like small GTPase promotes the binding of coat proteins onto the cytoplasmic domain of transmembrane cargo proteins to form a key intermediate that drives both cargo sorting and vesicle formation.	bind
44101	4	10172	7	NULL	NULL	0	NULL	statement 1	NULL		forms	NULL				key intermediate	NULL				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_168_2_281_s_8	15657398	A favored current model for how this coupling is achieved, known as the priming complex model ( ), proposes that the activated (GTP-bound) form of an ADP ribosylation factor (ARF) - like small GTPase promotes the binding of coat proteins onto the cytoplasmic domain of transmembrane cargo proteins to form a key intermediate that drives both cargo sorting and vesicle formation.	bind
44115	5	10172	7	NULL	NULL	0	NULL	statement 4	NULL		drives	NULL				cargo sorting	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_168_2_281_s_8	15657398	A favored current model for how this coupling is achieved, known as the priming complex model ( ), proposes that the activated (GTP-bound) form of an ADP ribosylation factor (ARF) - like small GTPase promotes the binding of coat proteins onto the cytoplasmic domain of transmembrane cargo proteins to form a key intermediate that drives both cargo sorting and vesicle formation.	bind
44116	6	10172	7	NULL	NULL	0	NULL	statement 4	NULL		drives	NULL				vesicle formation	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_168_2_281_s_8	15657398	A favored current model for how this coupling is achieved, known as the priming complex model ( ), proposes that the activated (GTP-bound) form of an ADP ribosylation factor (ARF) - like small GTPase promotes the binding of coat proteins onto the cytoplasmic domain of transmembrane cargo proteins to form a key intermediate that drives both cargo sorting and vesicle formation.	bind
44119	7	10172	7	NULL	NULL	0	NULL	ARF	NULL	activated	is	NULL				ADP ribosylation factor	NULL	GTP-bound form of			NULL		0	NULL	NULL	NULL	gw70_cellbiol_168_2_281_s_8	15657398	A favored current model for how this coupling is achieved, known as the priming complex model ( ), proposes that the activated (GTP-bound) form of an ADP ribosylation factor (ARF) - like small GTPase promotes the binding of coat proteins onto the cytoplasmic domain of transmembrane cargo proteins to form a key intermediate that drives both cargo sorting and vesicle formation.	bind
35895	1	10173	6	11	NULL	NULL	NULL	RepA initiator	GP		does not bind					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_26_5_533_s_140	12586394	A feature of Rep initiators is that, opposite to DnaA (see above), they do not  bind ATP.	bind
35896	2	10173	6	11	NULL	NULL	NULL	DnaA	GP		bind					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_26_5_533_s_140	12586394	A feature of Rep initiators is that, opposite to DnaA (see above), they do not  bind ATP.	bind
44127	1	10173	7	NULL	NULL	0	NULL	Rep initiators	NULL		does not bind	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_26_5_533_s_140	12586394	A feature of Rep initiators is that, opposite to DnaA (see above), they do not  bind ATP.	bind
44128	2	10173	7	NULL	NULL	0	NULL	DnaA	NULL		bind	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_26_5_533_s_140	12586394	A feature of Rep initiators is that, opposite to DnaA (see above), they do not  bind ATP.	bind
35899	1	10175	6	11	NULL	NULL	NULL	vWF	GP		bind					collagen	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_1_425_s_162	11756664	A feature that clearly distinguishes collagen-bound from self-assembled VWF multimers is the stability of interaction with the surface, because homotypic VWF interactions are reversible in a few minutes whereas VWF binding to collagen is apparently irreversible on a comparable time scale.	bind
35901	2	10175	6	11	NULL	NULL	NULL	vWF	GP		interacts with					vWF	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_1_425_s_162	11756664	A feature that clearly distinguishes collagen-bound from self-assembled VWF multimers is the stability of interaction with the surface, because homotypic VWF interactions are reversible in a few minutes whereas VWF binding to collagen is apparently irreversible on a comparable time scale.	bind
35912	3	10175	6	11	NULL	NULL	NULL	statement 1	Process		is reversible as compared to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_1_425_s_162	11756664	A feature that clearly distinguishes collagen-bound from self-assembled VWF multimers is the stability of interaction with the surface, because homotypic VWF interactions are reversible in a few minutes whereas VWF binding to collagen is apparently irreversible on a comparable time scale.	bind
44129	1	10175	7	NULL	NULL	0	NULL	VWF	NULL		bind	NULL				collagen	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_1_425_s_162	11756664	A feature that clearly distinguishes collagen-bound from self-assembled VWF multimers is the stability of interaction with the surface, because homotypic VWF interactions are reversible in a few minutes whereas VWF binding to collagen is apparently irreversible on a comparable time scale.	bind
44130	2	10175	7	10	NULL	0	NULL	vWF	NULL		interacts with	NULL				vWF	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_1_425_s_162	11756664	A feature that clearly distinguishes collagen-bound from self-assembled VWF multimers is the stability of interaction with the surface, because homotypic VWF interactions are reversible in a few minutes whereas VWF binding to collagen is apparently irreversible on a comparable time scale.	bind
44131	3	10175	7	10	NULL	0	NULL	statement 1	NULL		\tis reversible as compared to	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_1_425_s_162	11756664	A feature that clearly distinguishes collagen-bound from self-assembled VWF multimers is the stability of interaction with the surface, because homotypic VWF interactions are reversible in a few minutes whereas VWF binding to collagen is apparently irreversible on a comparable time scale.	bind
35965	1	10177	6	11	NULL	NULL	NULL	LDL	Chemical	plasma	bind					PBE-94	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0760-0779_biull-eksp-biol-med_110_9_2268712_s_2	2268712	A few alternatives of the binding of healthy patients plasma low density  lipoproteins (LDL) with anion exchanger PBE-94 were revealed.	bind
44134	1	10177	7	NULL	NULL	0	NULL	LDL	NULL	plasma	bind	NULL				PBE-94	NULL				NULL		0	NULL	NULL	NULL	abs-batch0760-0779_biull-eksp-biol-med_110_9_2268712_s_2	2268712	A few alternatives of the binding of healthy patients plasma low density  lipoproteins (LDL) with anion exchanger PBE-94 were revealed.	bind
35966	1	10178	6	11	NULL	NULL	NULL	nuclear factor I	GP		bind					alpha1(I) collagen	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_15_15639_s_19	14722113	A few common transcription factors such as nuclear factor I and Sp1 are known to bind and activate both the alpha1(I) ( ) and the alpha2(I) collagen promoters ( - ).	bind
35967	2	10178	6	11	NULL	NULL	NULL	statement 1	Process		activate					alpha1(I) collagen	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_15_15639_s_19	14722113	A few common transcription factors such as nuclear factor I and Sp1 are known to bind and activate both the alpha1(I) ( ) and the alpha2(I) collagen promoters ( - ).	bind
35968	3	10178	6	11	NULL	NULL	NULL	Sp1	GP		bind					alpha2(I) collagen	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_15_15639_s_19	14722113	A few common transcription factors such as nuclear factor I and Sp1 are known to bind and activate both the alpha1(I) ( ) and the alpha2(I) collagen promoters ( - ).	bind
35969	4	10178	6	11	NULL	NULL	NULL	statement 3	Process		activate					alpha2(I) collagen	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_15_15639_s_19	14722113	A few common transcription factors such as nuclear factor I and Sp1 are known to bind and activate both the alpha1(I) ( ) and the alpha2(I) collagen promoters ( - ).	bind
35970	5	10178	6	11	NULL	NULL	NULL	nuclear factor I	GP		bind					alpha2(I) collagen	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_15_15639_s_19	14722113	A few common transcription factors such as nuclear factor I and Sp1 are known to bind and activate both the alpha1(I) ( ) and the alpha2(I) collagen promoters ( - ).	bind
35971	6	10178	6	11	NULL	NULL	NULL	statement 5	Process		activate					alpha2(I) collagen	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_15_15639_s_19	14722113	A few common transcription factors such as nuclear factor I and Sp1 are known to bind and activate both the alpha1(I) ( ) and the alpha2(I) collagen promoters ( - ).	bind
35972	7	10178	6	11	NULL	NULL	NULL	Sp1	GP		bind					alpha1(I) collagen	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_15_15639_s_19	14722113	A few common transcription factors such as nuclear factor I and Sp1 are known to bind and activate both the alpha1(I) ( ) and the alpha2(I) collagen promoters ( - ).	bind
35973	8	10178	6	11	NULL	NULL	NULL	statement 7	Process		activates					alpha1(I) collagen	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_15_15639_s_19	14722113	A few common transcription factors such as nuclear factor I and Sp1 are known to bind and activate both the alpha1(I) ( ) and the alpha2(I) collagen promoters ( - ).	bind
35975	9	10178	6	11	NULL	NULL	NULL	Sp1	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_15_15639_s_19	14722113	A few common transcription factors such as nuclear factor I and Sp1 are known to bind and activate both the alpha1(I) ( ) and the alpha2(I) collagen promoters ( - ).	bind
35977	10	10178	6	11	NULL	NULL	NULL	nuclear factor I	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_15_15639_s_19	14722113	A few common transcription factors such as nuclear factor I and Sp1 are known to bind and activate both the alpha1(I) ( ) and the alpha2(I) collagen promoters ( - ).	bind
44135	1	10178	7	NULL	NULL	0	NULL	nuclear factor I 	NULL		bind	NULL				alpha1 collagen	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_15_15639_s_19	14722113	A few common transcription factors such as nuclear factor I and Sp1 are known to bind and activate both the alpha1(I) ( ) and the alpha2(I) collagen promoters ( - ).	bind
44136	2	10178	7	NULL	NULL	0	NULL	 nuclear factor I	NULL		bind	NULL				alpha2 collagen	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_15_15639_s_19	14722113	A few common transcription factors such as nuclear factor I and Sp1 are known to bind and activate both the alpha1(I) ( ) and the alpha2(I) collagen promoters ( - ).	bind
44137	3	10178	7	NULL	NULL	0	NULL	statement 1	NULL		activate	NULL				alpha1 collagen	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_15_15639_s_19	14722113	A few common transcription factors such as nuclear factor I and Sp1 are known to bind and activate both the alpha1(I) ( ) and the alpha2(I) collagen promoters ( - ).	bind
44138	4	10178	7	NULL	NULL	0	NULL	statement 2	NULL		activate	NULL				alpha2 collagen	NULL			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_15_15639_s_19	14722113	A few common transcription factors such as nuclear factor I and Sp1 are known to bind and activate both the alpha1(I) ( ) and the alpha2(I) collagen promoters ( - ).	bind
44139	5	10178	7	NULL	NULL	0	NULL	 Sp1	NULL		bind	NULL				alpha1 collagen	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_15_15639_s_19	14722113	A few common transcription factors such as nuclear factor I and Sp1 are known to bind and activate both the alpha1(I) ( ) and the alpha2(I) collagen promoters ( - ).	bind
44140	6	10178	7	NULL	NULL	0	NULL	Sp1	NULL		bind	NULL				alpha2 collagen	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_15_15639_s_19	14722113	A few common transcription factors such as nuclear factor I and Sp1 are known to bind and activate both the alpha1(I) ( ) and the alpha2(I) collagen promoters ( - ).	bind
44141	7	10178	7	NULL	NULL	0	NULL	statement 5	NULL		activate	NULL				alpha1 collagen	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_15_15639_s_19	14722113	A few common transcription factors such as nuclear factor I and Sp1 are known to bind and activate both the alpha1(I) ( ) and the alpha2(I) collagen promoters ( - ).	bind
44142	8	10178	7	NULL	NULL	0	NULL	statement 6	NULL		activate	NULL				alpha2 collagen	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_15_15639_s_19	14722113	A few common transcription factors such as nuclear factor I and Sp1 are known to bind and activate both the alpha1(I) ( ) and the alpha2(I) collagen promoters ( - ).	bind
49665	9	10178	7	10	NULL	0	NULL	Sp1	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_15_15639_s_19	14722113	A few common transcription factors such as nuclear factor I and Sp1 are known to bind and activate both the alpha1(I) ( ) and the alpha2(I) collagen promoters ( - ).	bind
49666	10	10178	7	10	NULL	0	NULL	nuclear factor I	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_15_15639_s_19	14722113	A few common transcription factors such as nuclear factor I and Sp1 are known to bind and activate both the alpha1(I) ( ) and the alpha2(I) collagen promoters ( - ).	bind
35979	1	10180	6	11	NULL	NULL	NULL	adenovirus	Organism		bind					vimentin	GP				NULL	HeLa cells	NULL	NULL	NULL	NULL	gw60_infectimmun_68_4_1787_s_278	10722565	A few examples of this have been observed, including the deleterious effects of adenovirus and human papillomavirus binding to vimentin and cytokeratins in HeLa cells and human keratinocytes, respectively ( 6,  47).	bind
35980	2	10180	6	11	NULL	NULL	NULL	papillomavirus	Organism	human	bind					cytokeratin	GP				NULL	human keratinocytes	NULL	NULL	NULL	NULL	gw60_infectimmun_68_4_1787_s_278	10722565	A few examples of this have been observed, including the deleterious effects of adenovirus and human papillomavirus binding to vimentin and cytokeratins in HeLa cells and human keratinocytes, respectively ( 6,  47).	bind
44143	1	10180	7	NULL	NULL	0	NULL	adenovirus	NULL		bind	NULL				vimentin	NULL				NULL	HeLa cells	NULL	NULL	NULL	NULL	gw60_infectimmun_68_4_1787_s_278	10722565	A few examples of this have been observed, including the deleterious effects of adenovirus and human papillomavirus binding to vimentin and cytokeratins in HeLa cells and human keratinocytes, respectively ( 6,  47).	bind
44150	2	10180	7	10	NULL	0	NULL	papillomavirus	NULL	human	bind	NULL				cytokeratins	NULL				NULL	human keratinocytes	NULL	NULL	NULL	NULL	gw60_infectimmun_68_4_1787_s_278	10722565	A few examples of this have been observed, including the deleterious effects of adenovirus and human papillomavirus binding to vimentin and cytokeratins in HeLa cells and human keratinocytes, respectively ( 6,  47).	bind
36103	1	10181	6	11	NULL	NULL	NULL	E1 tetramers	GP		bind					E2	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_69_0_961_s_611	10966480	A few molecules of kinase can rapidly inactivate the multiple E1 tetramers bound  to E2, and it has been proposed that the tightly bound kinase dimer may move by a  "`hand-over-hand"` mechanism around the surface of the E2 core, thereby encountering  (and phosphorylating) the E1  subunits, a process facilitated by the flexible linkers  in the E2p chain ( 147).	bind
37214	2	10181	6	11	NULL	NULL	NULL	kinase	GP		inactivate		rapidly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_69_0_961_s_611	10966480	A few molecules of kinase can rapidly inactivate the multiple E1 tetramers bound  to E2, and it has been proposed that the tightly bound kinase dimer may move by a  "`hand-over-hand"` mechanism around the surface of the E2 core, thereby encountering  (and phosphorylating) the E1  subunits, a process facilitated by the flexible linkers  in the E2p chain ( 147).	bind
37215	3	10181	6	11	NULL	NULL	NULL	kinase dimer	GP		bind		tightly			E2 core	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_69_0_961_s_611	10966480	A few molecules of kinase can rapidly inactivate the multiple E1 tetramers bound  to E2, and it has been proposed that the tightly bound kinase dimer may move by a  "`hand-over-hand"` mechanism around the surface of the E2 core, thereby encountering  (and phosphorylating) the E1  subunits, a process facilitated by the flexible linkers  in the E2p chain ( 147).	bind
37216	5	10181	6	11	NULL	NULL	NULL	statement 4	Process		encounter					E1 subunit	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_69_0_961_s_611	10966480	A few molecules of kinase can rapidly inactivate the multiple E1 tetramers bound  to E2, and it has been proposed that the tightly bound kinase dimer may move by a  "`hand-over-hand"` mechanism around the surface of the E2 core, thereby encountering  (and phosphorylating) the E1  subunits, a process facilitated by the flexible linkers  in the E2p chain ( 147).	bind
37217	6	10181	6	11	NULL	NULL	NULL	statement 5	GP		phosphorylates					E1 subunit	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_69_0_961_s_611	10966480	A few molecules of kinase can rapidly inactivate the multiple E1 tetramers bound  to E2, and it has been proposed that the tightly bound kinase dimer may move by a  "`hand-over-hand"` mechanism around the surface of the E2 core, thereby encountering  (and phosphorylating) the E1  subunits, a process facilitated by the flexible linkers  in the E2p chain ( 147).	bind
37305	4	10181	6	11	NULL	NULL	NULL	statement 3	GP		move around					E2 core	GP	surface of			NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_69_0_961_s_611	10966480	A few molecules of kinase can rapidly inactivate the multiple E1 tetramers bound  to E2, and it has been proposed that the tightly bound kinase dimer may move by a  "`hand-over-hand"` mechanism around the surface of the E2 core, thereby encountering  (and phosphorylating) the E1  subunits, a process facilitated by the flexible linkers  in the E2p chain ( 147).	bind
57479	7	10181	6	11	NULL	NULL	NULL	E2p chain	GP		facilitates			flexible linkers		statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_69_0_961_s_611	10966480	A few molecules of kinase can rapidly inactivate the multiple E1 tetramers bound  to E2, and it has been proposed that the tightly bound kinase dimer may move by a  "`hand-over-hand"` mechanism around the surface of the E2 core, thereby encountering  (and phosphorylating) the E1  subunits, a process facilitated by the flexible linkers  in the E2p chain ( 147).	bind
44151	1	10181	7	10	NULL	0	NULL	E1 tetramers			bind					E2					NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_69_0_961_s_611	10966480	A few molecules of kinase can rapidly inactivate the multiple E1 tetramers bound  to E2, and it has been proposed that the tightly bound kinase dimer may move by a  "`hand-over-hand"` mechanism around the surface of the E2 core, thereby encountering  (and phosphorylating) the E1  subunits, a process facilitated by the flexible linkers  in the E2p chain ( 147).	bind
44152	2	10181	7	NULL	NULL	0	NULL	kinase	NULL		inactivate	NULL	rapidly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_69_0_961_s_611	10966480	A few molecules of kinase can rapidly inactivate the multiple E1 tetramers bound  to E2, and it has been proposed that the tightly bound kinase dimer may move by a  "`hand-over-hand"` mechanism around the surface of the E2 core, thereby encountering  (and phosphorylating) the E1  subunits, a process facilitated by the flexible linkers  in the E2p chain ( 147).	bind
44153	3	10181	7	NULL	NULL	0	NULL	kinase dimer	NULL		bind	NULL	tightly			E2 core	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_69_0_961_s_611	10966480	A few molecules of kinase can rapidly inactivate the multiple E1 tetramers bound  to E2, and it has been proposed that the tightly bound kinase dimer may move by a  "`hand-over-hand"` mechanism around the surface of the E2 core, thereby encountering  (and phosphorylating) the E1  subunits, a process facilitated by the flexible linkers  in the E2p chain ( 147).	bind
44154	4	10181	7	NULL	NULL	0	NULL	statement 3	NULL		move around	NULL				E2 core	NULL	surface of			NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_69_0_961_s_611	10966480	A few molecules of kinase can rapidly inactivate the multiple E1 tetramers bound  to E2, and it has been proposed that the tightly bound kinase dimer may move by a  "`hand-over-hand"` mechanism around the surface of the E2 core, thereby encountering  (and phosphorylating) the E1  subunits, a process facilitated by the flexible linkers  in the E2p chain ( 147).	bind
44155	6	10181	7	10	NULL	0	NULL	statement 5			phosphorylate					E1 subunits					NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_69_0_961_s_611	10966480	A few molecules of kinase can rapidly inactivate the multiple E1 tetramers bound  to E2, and it has been proposed that the tightly bound kinase dimer may move by a  "`hand-over-hand"` mechanism around the surface of the E2 core, thereby encountering  (and phosphorylating) the E1  subunits, a process facilitated by the flexible linkers  in the E2p chain ( 147).	bind
44156	7	10181	7	10	NULL	0	NULL	E2p chain			facilitate			flexible linkers		statement 6					NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_69_0_961_s_611	10966480	A few molecules of kinase can rapidly inactivate the multiple E1 tetramers bound  to E2, and it has been proposed that the tightly bound kinase dimer may move by a  "`hand-over-hand"` mechanism around the surface of the E2 core, thereby encountering  (and phosphorylating) the E1  subunits, a process facilitated by the flexible linkers  in the E2p chain ( 147).	bind
44157	5	10181	7	10	NULL	0	NULL	statement 4			encounter					E1 subunits					NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_69_0_961_s_611	10966480	A few molecules of kinase can rapidly inactivate the multiple E1 tetramers bound  to E2, and it has been proposed that the tightly bound kinase dimer may move by a  "`hand-over-hand"` mechanism around the surface of the E2 core, thereby encountering  (and phosphorylating) the E1  subunits, a process facilitated by the flexible linkers  in the E2p chain ( 147).	bind
35981	1	10182	6	11	NULL	NULL	NULL	HFE	GP		bind					transferrin receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_18_2_205_s_210	12594948	A few perform unrelated functions, however, such as HFE, which binds to the transferrin receptor and regulates iron homeostasis  (Feder et al., 1998  ).	bind
35982	2	10182	6	11	NULL	NULL	NULL	statement 1	Process		regulates					iron	Chemical	homeostasis of 			NULL		NULL	NULL	NULL	NULL	gw60_immunity_18_2_205_s_210	12594948	A few perform unrelated functions, however, such as HFE, which binds to the transferrin receptor and regulates iron homeostasis  (Feder et al., 1998  ).	bind
44158	1	10182	7	NULL	NULL	0	NULL	HFE	NULL		binds to	NULL				transferrin receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_immunity_18_2_205_s_210	12594948	A few perform unrelated functions, however, such as HFE, which binds to the transferrin receptor and regulates iron homeostasis  (Feder et al., 1998  ).	bind
44159	2	10182	7	10	NULL	0	NULL	statement 1	NULL		regulates	NULL				iron	NULL	homeostasis of			NULL		NULL	NULL	NULL	NULL	gw60_immunity_18_2_205_s_210	12594948	A few perform unrelated functions, however, such as HFE, which binds to the transferrin receptor and regulates iron homeostasis  (Feder et al., 1998  ).	bind
35983	1	10183	6	11	NULL	NULL	NULL	RPL3	GP		is 					ribosomal protein L3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2066_s_294	10688653	A few ribosomal protein genes, including  RPL3 (encoding ribosomal protein L3), have no site for Rap1 but have a single Abf1-binding site instead ( 3,  6,  8).	bind
35984	2	10183	6	11	NULL	NULL	NULL	RPL3	GP		have no site for					Rap1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2066_s_294	10688653	A few ribosomal protein genes, including  RPL3 (encoding ribosomal protein L3), have no site for Rap1 but have a single Abf1-binding site instead ( 3,  6,  8).	bind
35985	3	10183	6	11	NULL	NULL	NULL	RPL3	GP		have 							single		Abf1-binding site	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2066_s_294	10688653	A few ribosomal protein genes, including  RPL3 (encoding ribosomal protein L3), have no site for Rap1 but have a single Abf1-binding site instead ( 3,  6,  8).	bind
44160	1	10183	7	10	NULL	0	NULL	RPL3 	NULL		contains	NULL					NULL			Abf1-binding site	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2066_s_294	10688653	A few ribosomal protein genes, including  RPL3 (encoding ribosomal protein L3), have no site for Rap1 but have a single Abf1-binding site instead ( 3,  6,  8).	bind
44161	2	10183	7	NULL	NULL	0	NULL	RPL3	NULL		is	NULL				encoding ribosomal protein L3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2066_s_294	10688653	A few ribosomal protein genes, including  RPL3 (encoding ribosomal protein L3), have no site for Rap1 but have a single Abf1-binding site instead ( 3,  6,  8).	bind
44162	3	10183	7	10	NULL	0	NULL	RPL3	NULL		have no site for	NULL				Rap1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2066_s_294	10688653	A few ribosomal protein genes, including  RPL3 (encoding ribosomal protein L3), have no site for Rap1 but have a single Abf1-binding site instead ( 3,  6,  8).	bind
35989	1	10185	6	11	NULL	NULL	NULL	EBP2	GP	human	bind		specifically			EBNA1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_4934_s_18	15923612	A few years ago, we identified a previously uncharacterized cellular protein that we called EBNA1 binding protein 2 (EBP2) from a two-hybrid screening for human proteins that specifically bind EBNA1 ( ).	bind
35990	2	10185	6	11	NULL	NULL	NULL	EBP2	GP		is					EBNA1 binding protein 2 	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_4934_s_18	15923612	A few years ago, we identified a previously uncharacterized cellular protein that we called EBNA1 binding protein 2 (EBP2) from a two-hybrid screening for human proteins that specifically bind EBNA1 ( ).	bind
44164	1	10185	7	10	NULL	0	NULL	EBP2	NULL	human	bind	NULL	specifically			EBNA1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_4934_s_18	15923612	A few years ago, we identified a previously uncharacterized cellular protein that we called EBNA1 binding protein 2 (EBP2) from a two-hybrid screening for human proteins that specifically bind EBNA1 ( ).	bind
44165	2	10185	7	NULL	NULL	0	NULL	EBP2	NULL		is	NULL				EBNA1 binding protein 2	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_12_4934_s_18	15923612	A few years ago, we identified a previously uncharacterized cellular protein that we called EBNA1 binding protein 2 (EBP2) from a two-hybrid screening for human proteins that specifically bind EBNA1 ( ).	bind
35992	1	10186	6	11	NULL	NULL	NULL	FAP	GP	M. avium	bind		may			fibronectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_microbesinfect_3_1_37_s_37	11226852	A fibronectin attachment protein (FAP) has been described on  M. avium and it has been hypothesized that FAP would bind fibronectin that could work as a bridge between the bacterial and the mucosal cell.	bind
35993	2	10186	6	11	NULL	NULL	NULL	FAP	GP		is					fibronectin attachment protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_microbesinfect_3_1_37_s_37	11226852	A fibronectin attachment protein (FAP) has been described on  M. avium and it has been hypothesized that FAP would bind fibronectin that could work as a bridge between the bacterial and the mucosal cell.	bind
36301	3	10186	6	11	NULL	NULL	NULL	bacterial cell	Organism		bridge between					mucosal cell	Cell				NULL		NULL	NULL	NULL	NULL	gw60_microbesinfect_3_1_37_s_37	11226852	A fibronectin attachment protein (FAP) has been described on  M. avium and it has been hypothesized that FAP would bind fibronectin that could work as a bridge between the bacterial and the mucosal cell.	bind
36302	4	10186	6	11	NULL	NULL	NULL	statement 1	Process		leads to		may			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_microbesinfect_3_1_37_s_37	11226852	A fibronectin attachment protein (FAP) has been described on  M. avium and it has been hypothesized that FAP would bind fibronectin that could work as a bridge between the bacterial and the mucosal cell.	bind
44166	1	10186	7	10	NULL	0	NULL	FAP		M. avium	bind		may			fibronectin					NULL		NULL	NULL	NULL	NULL	gw60_microbesinfect_3_1_37_s_37	11226852	A fibronectin attachment protein (FAP) has been described on  M. avium and it has been hypothesized that FAP would bind fibronectin that could work as a bridge between the bacterial and the mucosal cell.	bind
44167	2	10186	7	NULL	NULL	0	NULL	FAP	NULL		is	NULL				fibronectin attachment protein	NULL				NULL		0	NULL	NULL	NULL	gw60_microbesinfect_3_1_37_s_37	11226852	A fibronectin attachment protein (FAP) has been described on  M. avium and it has been hypothesized that FAP would bind fibronectin that could work as a bridge between the bacterial and the mucosal cell.	bind
44182	3	10186	7	NULL	NULL	0	NULL	bacterial cell	NULL		bridge between	NULL				mucosal cell	NULL				NULL		0	NULL	NULL	NULL	gw60_microbesinfect_3_1_37_s_37	11226852	A fibronectin attachment protein (FAP) has been described on  M. avium and it has been hypothesized that FAP would bind fibronectin that could work as a bridge between the bacterial and the mucosal cell.	bind
44183	4	10186	7	10	NULL	0	NULL	statement 1			leads to		may			statement 3					NULL		NULL	NULL	NULL	NULL	gw60_microbesinfect_3_1_37_s_37	11226852	A fibronectin attachment protein (FAP) has been described on  M. avium and it has been hypothesized that FAP would bind fibronectin that could work as a bridge between the bacterial and the mucosal cell.	bind
35994	1	10187	6	11	NULL	NULL	NULL	fibronectin-binding protein	GP	Streptococcus equi	bind					collagen	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_biochem-biophys-res-commun_340_2_16376297_s_1	16376297	A fibronectin-binding protein from Streptococcus equi binds collagen and modulates cell-mediated collagen gel contraction..	bind
35995	2	10187	6	11	NULL	NULL	NULL	cell	Cell		mediates					collagen gel 	GP	contraction of			NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_biochem-biophys-res-commun_340_2_16376297_s_1	16376297	A fibronectin-binding protein from Streptococcus equi binds collagen and modulates cell-mediated collagen gel contraction..	bind
49667	3	10187	6	11	NULL	NULL	NULL	statement 1	Process		modulates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_biochem-biophys-res-commun_340_2_16376297_s_1	16376297	A fibronectin-binding protein from Streptococcus equi binds collagen and modulates cell-mediated collagen gel contraction..	bind
44184	1	10187	7	NULL	NULL	0	NULL	fibronectin-binding protein	NULL	Streptococcus equi	binds	NULL				collagen	NULL				NULL		0	NULL	NULL	NULL	abs-batch0570-0579_biochem-biophys-res-commun_340_2_16376297_s_1	16376297	A fibronectin-binding protein from Streptococcus equi binds collagen and modulates cell-mediated collagen gel contraction..	bind
44185	2	10187	7	NULL	NULL	0	NULL	cell	NULL		mediates	NULL				collagen gel 	NULL	contraction of			NULL		0	NULL	NULL	NULL	abs-batch0570-0579_biochem-biophys-res-commun_340_2_16376297_s_1	16376297	A fibronectin-binding protein from Streptococcus equi binds collagen and modulates cell-mediated collagen gel contraction..	bind
44186	3	10187	7	NULL	NULL	0	NULL	statement 1	NULL		modulates	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	abs-batch0570-0579_biochem-biophys-res-commun_340_2_16376297_s_1	16376297	A fibronectin-binding protein from Streptococcus equi binds collagen and modulates cell-mediated collagen gel contraction..	bind
35997	1	10189	6	11	NULL	NULL	NULL	HGFSF	GP	wt	bind					heparin	Chemical	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_3_125_s_280	9443912	A figure showing BIAcore analysis of wt-HGFSF and HP1 binding to immobilised heparin is published with this paper on the internet.	bind
35999	2	10189	6	11	NULL	NULL	NULL	HP1	GP		bind					heparin	Chemical	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_3_125_s_280	9443912	A figure showing BIAcore analysis of wt-HGFSF and HP1 binding to immobilised heparin is published with this paper on the internet.	bind
44188	1	10189	7	NULL	NULL	0	NULL	HGFSF	NULL	wt	bind	NULL				heparin	NULL	immobilized			NULL		0	NULL	NULL	NULL	gw60_currbiol_8_3_125_s_280	9443912	A figure showing BIAcore analysis of wt-HGFSF and HP1 binding to immobilised heparin is published with this paper on the internet.	bind
44189	2	10189	7	NULL	NULL	0	NULL	HP1	NULL		bind	NULL				heparin	NULL	immobilized			NULL		0	NULL	NULL	NULL	gw60_currbiol_8_3_125_s_280	9443912	A figure showing BIAcore analysis of wt-HGFSF and HP1 binding to immobilised heparin is published with this paper on the internet.	bind
36016	1	10190	6	11	NULL	NULL	NULL	[125]E r-1	GP		bind					p143	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_4_1445_s_184	10749941	A filled arrowhead indicates [125]E r-1 binding to p143.	bind
44190	1	10190	7	NULL	NULL	0	NULL	[125]E r-1	NULL		bind	NULL				p143	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1445_s_184	10749941	A filled arrowhead indicates [125]E r-1 binding to p143.	bind
36017	1	10191	6	11	NULL	NULL	NULL	AnCOB protein extract	GP		bind		tightly			AnCOB precursor	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_17_8994_s_130	9256423	A filter binding assay (Fig.  4) showed that the AnCOB protein extract bound tightly to the AnCOB precursor ( Kd = 3 nM) and very poorly to a precursor containing the AnOX2 intron.	bind
36018	2	10191	6	11	NULL	NULL	NULL	AnCOB protein extract	GP		bind		poorly			AnOX2 intron precursor	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_17_8994_s_130	9256423	A filter binding assay (Fig.  4) showed that the AnCOB protein extract bound tightly to the AnCOB precursor ( Kd = 3 nM) and very poorly to a precursor containing the AnOX2 intron.	bind
44191	1	10191	7	NULL	NULL	0	NULL	AnCOB protein extract	NULL		bind	NULL	tightly			AnCOB precursor	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_94_17_8994_s_130	9256423	A filter binding assay (Fig.  4) showed that the AnCOB protein extract bound tightly to the AnCOB precursor ( Kd = 3 nM) and very poorly to a precursor containing the AnOX2 intron.	bind
44192	2	10191	7	10	NULL	0	NULL	 AnCOB protein extract			bind		poorly			 AnOX2 intron precursor					NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_17_8994_s_130	9256423	A filter binding assay (Fig.  4) showed that the AnCOB protein extract bound tightly to the AnCOB precursor ( Kd = 3 nM) and very poorly to a precursor containing the AnOX2 intron.	bind
36020	1	10192	6	11	NULL	NULL	NULL	ATP	Chemical		bind					MutL	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_97_1_85_s_224	10199405	A filter binding assay using  - and  -32P-labeled  ATP that allows quantitation of the amounts of ATP and ADP bound  to MutL was employed to study the dynamics of nucleotide - protein interaction and  the rate-limiting step of ATP hydrolysis (see Experimental Procedures).	bind
36021	2	10192	6	11	NULL	NULL	NULL	ADP	Chemical		bind					MutL	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_97_1_85_s_224	10199405	A filter binding assay using  - and  -32P-labeled  ATP that allows quantitation of the amounts of ATP and ADP bound  to MutL was employed to study the dynamics of nucleotide - protein interaction and  the rate-limiting step of ATP hydrolysis (see Experimental Procedures).	bind
44198	1	10192	7	NULL	NULL	0	NULL	ATP	NULL		bind	NULL				MutL	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_97_1_85_s_224	10199405	A filter binding assay using  - and  -32P-labeled  ATP that allows quantitation of the amounts of ATP and ADP bound  to MutL was employed to study the dynamics of nucleotide - protein interaction and  the rate-limiting step of ATP hydrolysis (see Experimental Procedures).	bind
44199	2	10192	7	NULL	NULL	0	NULL	ADP	NULL		bind	NULL				MutL	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_97_1_85_s_224	10199405	A filter binding assay using  - and  -32P-labeled  ATP that allows quantitation of the amounts of ATP and ADP bound  to MutL was employed to study the dynamics of nucleotide - protein interaction and  the rate-limiting step of ATP hydrolysis (see Experimental Procedures).	bind
36022	1	10193	6	11	NULL	NULL	NULL	4.5 RNA	NucleicAcid		bind					Ffh	GP	purified			NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_180_2_271_s_102	10556722	A filter binding assay using purified Ffh and EF-G (1-91) confirmed in this study that the binding affinity of 4.5 RNA for Ffh and EF-G is quite different.	bind
36023	2	10193	6	11	NULL	NULL	NULL	4.5 RNA	NucleicAcid		bind					EF-G	GP	purified			NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_180_2_271_s_102	10556722	A filter binding assay using purified Ffh and EF-G (1-91) confirmed in this study that the binding affinity of 4.5 RNA for Ffh and EF-G is quite different.	bind
49669	3	10193	6	11	NULL	NULL	NULL	statement 1	Process	affinity of	is different from					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_180_2_271_s_102	10556722	A filter binding assay using purified Ffh and EF-G (1-91) confirmed in this study that the binding affinity of 4.5 RNA for Ffh and EF-G is quite different.	bind
44200	1	10193	7	NULL	NULL	0	NULL	Ffh	NULL	purified	bind	NULL				4.5RNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_180_2_271_s_102	10556722	A filter binding assay using purified Ffh and EF-G (1-91) confirmed in this study that the binding affinity of 4.5 RNA for Ffh and EF-G is quite different.	bind
44201	2	10193	7	NULL	NULL	0	NULL	EF-G	NULL	purified	bind	NULL				4.5RNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_180_2_271_s_102	10556722	A filter binding assay using purified Ffh and EF-G (1-91) confirmed in this study that the binding affinity of 4.5 RNA for Ffh and EF-G is quite different.	bind
44202	3	10193	7	10	NULL	0	NULL	statement 1	NULL	affinity of	is different from	NULL				statement 2	NULL	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_180_2_271_s_102	10556722	A filter binding assay using purified Ffh and EF-G (1-91) confirmed in this study that the binding affinity of 4.5 RNA for Ffh and EF-G is quite different.	bind
36024	1	10194	6	11	NULL	NULL	NULL	trp repressor	GP		bind		specifically			DNA	NucleicAcid			operator	NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_nucleic-acids-res_15_13_3299270_s_2	3299270	A filter binding assay was developed that allows measurement of specific  binding of trp repressor to operator DNA.	bind
44205	1	10194	7	NULL	NULL	0	NULL	trp repressor	NULL		bind	NULL	specifically			DNA	NULL			operator	NULL		0	NULL	NULL	NULL	abs-batch0650-0679_nucleic-acids-res_15_13_3299270_s_2	3299270	A filter binding assay was developed that allows measurement of specific  binding of trp repressor to operator DNA.	bind
36026	1	10196	6	11	NULL	NULL	NULL	VDR/RXR heterodimer	GP		bind					TRPV6 gene	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_mol-endocrinol_20_6_16574738_s_11	16574738	A final  ChIP assay revealed that VDR/RXR heterodimer binding to the TRPV6 gene  was accompanied by both the recruitment of steroid receptor coactivator  1 as well as a broad change in histone 4 acetylation.	bind
36027	2	10196	6	11	NULL	NULL	NULL	statement 1	Process		occurs by					steroid receptor coactivator 1	GP	recruitment of			NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_mol-endocrinol_20_6_16574738_s_11	16574738	A final  ChIP assay revealed that VDR/RXR heterodimer binding to the TRPV6 gene  was accompanied by both the recruitment of steroid receptor coactivator  1 as well as a broad change in histone 4 acetylation.	bind
36028	3	10196	6	11	NULL	NULL	NULL	statement 1	Process		occurs by					histone 4	GP	change in acetylation of			NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_mol-endocrinol_20_6_16574738_s_11	16574738	A final  ChIP assay revealed that VDR/RXR heterodimer binding to the TRPV6 gene  was accompanied by both the recruitment of steroid receptor coactivator  1 as well as a broad change in histone 4 acetylation.	bind
36030	4	10196	6	11	NULL	NULL	NULL	statement 2	Process		occurs simultaneously with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_mol-endocrinol_20_6_16574738_s_11	16574738	A final  ChIP assay revealed that VDR/RXR heterodimer binding to the TRPV6 gene  was accompanied by both the recruitment of steroid receptor coactivator  1 as well as a broad change in histone 4 acetylation.	bind
44206	1	10196	7	NULL	NULL	0	NULL	VDR/RXR heterodimer	NULL		bind	NULL				TRPV6 gene	NULL				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_mol-endocrinol_20_6_16574738_s_11	16574738	A final  ChIP assay revealed that VDR/RXR heterodimer binding to the TRPV6 gene  was accompanied by both the recruitment of steroid receptor coactivator  1 as well as a broad change in histone 4 acetylation.	bind
44207	2	10196	7	NULL	NULL	0	NULL	statement 1	NULL		recruits	NULL				steroid receptor coactivator 1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_mol-endocrinol_20_6_16574738_s_11	16574738	A final  ChIP assay revealed that VDR/RXR heterodimer binding to the TRPV6 gene  was accompanied by both the recruitment of steroid receptor coactivator  1 as well as a broad change in histone 4 acetylation.	bind
44208	3	10196	7	NULL	NULL	0	NULL	statement 1	NULL		changes	NULL				histone 4	NULL	acetylation of			NULL		0	NULL	NULL	NULL	abs-batch0700-0719_mol-endocrinol_20_6_16574738_s_11	16574738	A final  ChIP assay revealed that VDR/RXR heterodimer binding to the TRPV6 gene  was accompanied by both the recruitment of steroid receptor coactivator  1 as well as a broad change in histone 4 acetylation.	bind
57480	4	10196	7	10	NULL	0	NULL	statement 2			occurs simultaneously with					statement 3					NULL		0	NULL	NULL	NULL	abs-batch0700-0719_mol-endocrinol_20_6_16574738_s_11	16574738	A final  ChIP assay revealed that VDR/RXR heterodimer binding to the TRPV6 gene  was accompanied by both the recruitment of steroid receptor coactivator  1 as well as a broad change in histone 4 acetylation.	bind
36031	1	10197	6	11	NULL	NULL	NULL	Rab11-FIP1	GP		bind					Rab11a	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_39067_s_343	11495908	A final explanation is that Rab11-FIP1, Rab11-FIP2, Rab11-FIP3, and pp75/Rip11 all bind Rab11a, Rab11b, or Rab25, but their binding may be reserved for different functions oriented in time.	bind
36032	2	10197	6	11	NULL	NULL	NULL	Rab11-FIP1	GP		bind					Rab11b	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_39067_s_343	11495908	A final explanation is that Rab11-FIP1, Rab11-FIP2, Rab11-FIP3, and pp75/Rip11 all bind Rab11a, Rab11b, or Rab25, but their binding may be reserved for different functions oriented in time.	bind
36033	3	10197	6	11	NULL	NULL	NULL	Rab11-FIP1	GP		bind					Rab25	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_39067_s_343	11495908	A final explanation is that Rab11-FIP1, Rab11-FIP2, Rab11-FIP3, and pp75/Rip11 all bind Rab11a, Rab11b, or Rab25, but their binding may be reserved for different functions oriented in time.	bind
36034	4	10197	6	11	NULL	NULL	NULL	Rab11-FIP2	GP		bind					Rab11a	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_39067_s_343	11495908	A final explanation is that Rab11-FIP1, Rab11-FIP2, Rab11-FIP3, and pp75/Rip11 all bind Rab11a, Rab11b, or Rab25, but their binding may be reserved for different functions oriented in time.	bind
36036	5	10197	6	11	NULL	NULL	NULL	Rab11-FIP2	GP		bind					Rab11b	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_39067_s_343	11495908	A final explanation is that Rab11-FIP1, Rab11-FIP2, Rab11-FIP3, and pp75/Rip11 all bind Rab11a, Rab11b, or Rab25, but their binding may be reserved for different functions oriented in time.	bind
36038	6	10197	6	11	NULL	NULL	NULL	Rab11-FIP2	GP		bind					Rab25	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_39067_s_343	11495908	A final explanation is that Rab11-FIP1, Rab11-FIP2, Rab11-FIP3, and pp75/Rip11 all bind Rab11a, Rab11b, or Rab25, but their binding may be reserved for different functions oriented in time.	bind
36039	7	10197	6	11	NULL	NULL	NULL	Rab11-FIP3	GP		bind					Rab11a	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_39067_s_343	11495908	A final explanation is that Rab11-FIP1, Rab11-FIP2, Rab11-FIP3, and pp75/Rip11 all bind Rab11a, Rab11b, or Rab25, but their binding may be reserved for different functions oriented in time.	bind
36040	8	10197	6	11	NULL	NULL	NULL	Rab11-FIP3	GP		bind					Rab11b	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_39067_s_343	11495908	A final explanation is that Rab11-FIP1, Rab11-FIP2, Rab11-FIP3, and pp75/Rip11 all bind Rab11a, Rab11b, or Rab25, but their binding may be reserved for different functions oriented in time.	bind
36041	9	10197	6	11	NULL	NULL	NULL	Rab11-FIP3	GP		bind					Rab25	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_39067_s_343	11495908	A final explanation is that Rab11-FIP1, Rab11-FIP2, Rab11-FIP3, and pp75/Rip11 all bind Rab11a, Rab11b, or Rab25, but their binding may be reserved for different functions oriented in time.	bind
36043	10	10197	6	11	NULL	NULL	NULL	pp75/Rip11	GP		bind					Rab11a	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_39067_s_343	11495908	A final explanation is that Rab11-FIP1, Rab11-FIP2, Rab11-FIP3, and pp75/Rip11 all bind Rab11a, Rab11b, or Rab25, but their binding may be reserved for different functions oriented in time.	bind
36044	11	10197	6	11	NULL	NULL	NULL	pp75/Rip11	GP		bind					Rab11b	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_39067_s_343	11495908	A final explanation is that Rab11-FIP1, Rab11-FIP2, Rab11-FIP3, and pp75/Rip11 all bind Rab11a, Rab11b, or Rab25, but their binding may be reserved for different functions oriented in time.	bind
36046	12	10197	6	11	NULL	NULL	NULL	pp75/Rip11	GP		bind					Rab25	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_39067_s_343	11495908	A final explanation is that Rab11-FIP1, Rab11-FIP2, Rab11-FIP3, and pp75/Rip11 all bind Rab11a, Rab11b, or Rab25, but their binding may be reserved for different functions oriented in time.	bind
44209	1	10197	7	NULL	NULL	0	NULL	Rab11-FIP1	NULL		bind	NULL				Rab11a	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_39067_s_343	11495908	A final explanation is that Rab11-FIP1, Rab11-FIP2, Rab11-FIP3, and pp75/Rip11 all bind Rab11a, Rab11b, or Rab25, but their binding may be reserved for different functions oriented in time.	bind
44210	2	10197	7	NULL	NULL	0	NULL	Rab11-FIP1	NULL		bind	NULL				Rab11b	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_39067_s_343	11495908	A final explanation is that Rab11-FIP1, Rab11-FIP2, Rab11-FIP3, and pp75/Rip11 all bind Rab11a, Rab11b, or Rab25, but their binding may be reserved for different functions oriented in time.	bind
44211	3	10197	7	NULL	NULL	0	NULL	Rab11-FIP1	NULL		bind	NULL				Rab25	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_39067_s_343	11495908	A final explanation is that Rab11-FIP1, Rab11-FIP2, Rab11-FIP3, and pp75/Rip11 all bind Rab11a, Rab11b, or Rab25, but their binding may be reserved for different functions oriented in time.	bind
44261	4	10197	7	NULL	NULL	0	NULL	Rab11-FIP2	NULL		bind	NULL				Rab11a	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_39067_s_343	11495908	A final explanation is that Rab11-FIP1, Rab11-FIP2, Rab11-FIP3, and pp75/Rip11 all bind Rab11a, Rab11b, or Rab25, but their binding may be reserved for different functions oriented in time.	bind
44262	5	10197	7	NULL	NULL	0	NULL	Rab11-FIP2	NULL		bind	NULL				Rab11b	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_39067_s_343	11495908	A final explanation is that Rab11-FIP1, Rab11-FIP2, Rab11-FIP3, and pp75/Rip11 all bind Rab11a, Rab11b, or Rab25, but their binding may be reserved for different functions oriented in time.	bind
44263	6	10197	7	NULL	NULL	0	NULL	Rab11-FIP2	NULL		bind	NULL				Rab25	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_39067_s_343	11495908	A final explanation is that Rab11-FIP1, Rab11-FIP2, Rab11-FIP3, and pp75/Rip11 all bind Rab11a, Rab11b, or Rab25, but their binding may be reserved for different functions oriented in time.	bind
44264	7	10197	7	NULL	NULL	0	NULL	Rab11-FIP3	NULL		bind	NULL				Rab11a	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_39067_s_343	11495908	A final explanation is that Rab11-FIP1, Rab11-FIP2, Rab11-FIP3, and pp75/Rip11 all bind Rab11a, Rab11b, or Rab25, but their binding may be reserved for different functions oriented in time.	bind
44265	8	10197	7	NULL	NULL	0	NULL	Rab11-FIP3	NULL		bind	NULL				Rab11b	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_39067_s_343	11495908	A final explanation is that Rab11-FIP1, Rab11-FIP2, Rab11-FIP3, and pp75/Rip11 all bind Rab11a, Rab11b, or Rab25, but their binding may be reserved for different functions oriented in time.	bind
44266	9	10197	7	NULL	NULL	0	NULL	Rab11-FIP3	NULL		bind	NULL				Rab25	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_39067_s_343	11495908	A final explanation is that Rab11-FIP1, Rab11-FIP2, Rab11-FIP3, and pp75/Rip11 all bind Rab11a, Rab11b, or Rab25, but their binding may be reserved for different functions oriented in time.	bind
44271	10	10197	7	NULL	NULL	0	NULL	pp75/Rip11	NULL		bind	NULL				Rab11a	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_39067_s_343	11495908	A final explanation is that Rab11-FIP1, Rab11-FIP2, Rab11-FIP3, and pp75/Rip11 all bind Rab11a, Rab11b, or Rab25, but their binding may be reserved for different functions oriented in time.	bind
44272	11	10197	7	NULL	NULL	0	NULL	pp75/Rip11	NULL		bind	NULL				Rab11b	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_39067_s_343	11495908	A final explanation is that Rab11-FIP1, Rab11-FIP2, Rab11-FIP3, and pp75/Rip11 all bind Rab11a, Rab11b, or Rab25, but their binding may be reserved for different functions oriented in time.	bind
44273	12	10197	7	NULL	NULL	0	NULL	pp75/Rip11	NULL		bind	NULL				Rab25	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_39067_s_343	11495908	A final explanation is that Rab11-FIP1, Rab11-FIP2, Rab11-FIP3, and pp75/Rip11 all bind Rab11a, Rab11b, or Rab25, but their binding may be reserved for different functions oriented in time.	bind
36050	1	10200	6	11	NULL	NULL	NULL	intimin-alpha	GP		contains		may			host cell surface receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2876_s_44	11704679	A final line of evidence that suggests that intimin may have a host cell surface receptor other than Tir comes from mutational analysis of the host cell binding domain of intimin-alpha.	bind
49668	2	10200	6	11	NULL	NULL	NULL	intimin	GP		contains					Tir	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2876_s_44	11704679	A final line of evidence that suggests that intimin may have a host cell surface receptor other than Tir comes from mutational analysis of the host cell binding domain of intimin-alpha.	bind
44276	1	10200	7	10	NULL	0	NULL	intimin-alpha	NULL		contains	NULL	may			host cell surface receptor	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2876_s_44	11704679	A final line of evidence that suggests that intimin may have a host cell surface receptor other than Tir comes from mutational analysis of the host cell binding domain of intimin-alpha.	bind
44277	2	10200	7	NULL	NULL	0	NULL	intimin	NULL		contains	NULL				Tir	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2876_s_44	11704679	A final line of evidence that suggests that intimin may have a host cell surface receptor other than Tir comes from mutational analysis of the host cell binding domain of intimin-alpha.	bind
43388	1	10201	5	11	NULL	NULL	NULL	md130	Organism	mutation	does not affect		possibly			VA	MedicalProcedure	binding of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_5_2479_s_204	10051668	A final possibility is that the  md130 mutation does not affect VA binding; rather, it could indirectly decrease VA efficacy by counteracting the effect of VA binding or regulate the process disrupted by VAs.	bind
43389	2	10201	5	11	NULL	NULL	NULL	md130	Organism	mutation	counteracts		possibly			VA	MedicalProcedure	effect of;;binding of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_5_2479_s_204	10051668	A final possibility is that the  md130 mutation does not affect VA binding; rather, it could indirectly decrease VA efficacy by counteracting the effect of VA binding or regulate the process disrupted by VAs.	bind
43390	3	10201	5	11	NULL	NULL	NULL	md130	Organism	mutation	decrease		indirectly;;possibly			VA	MedicalProcedure	efficacy of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_5_2479_s_204	10051668	A final possibility is that the  md130 mutation does not affect VA binding; rather, it could indirectly decrease VA efficacy by counteracting the effect of VA binding or regulate the process disrupted by VAs.	bind
43393	4	10201	5	11	NULL	NULL	NULL	statement 2	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_5_2479_s_204	10051668	A final possibility is that the  md130 mutation does not affect VA binding; rather, it could indirectly decrease VA efficacy by counteracting the effect of VA binding or regulate the process disrupted by VAs.	bind
36330	1	10201	6	10	NULL	0	NULL	md130		mutation of	does not affect		possibly			VA		binding of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_5_2479_s_204	10051668	A final possibility is that the  md130 mutation does not affect VA binding; rather, it could indirectly decrease VA efficacy by counteracting the effect of VA binding or regulate the process disrupted by VAs.	bind
57481	2	10201	6	10	NULL	0	NULL	md130		mutation of	counteracts		possibly			VA		effect of;;binding of			NULL		0	NULL	NULL	NULL	gw60_pnas_96_5_2479_s_204	10051668	A final possibility is that the  md130 mutation does not affect VA binding; rather, it could indirectly decrease VA efficacy by counteracting the effect of VA binding or regulate the process disrupted by VAs.	bind
57482	3	10201	6	10	NULL	0	NULL	md130		mutation of	decrease		indirectly;;possibly \t			VA		efficacy of			NULL		0	NULL	NULL	NULL	gw60_pnas_96_5_2479_s_204	10051668	A final possibility is that the  md130 mutation does not affect VA binding; rather, it could indirectly decrease VA efficacy by counteracting the effect of VA binding or regulate the process disrupted by VAs.	bind
57483	4	10201	6	10	NULL	0	NULL	statement 2			leads to					statement 3					NULL		0	NULL	NULL	NULL	gw60_pnas_96_5_2479_s_204	10051668	A final possibility is that the  md130 mutation does not affect VA binding; rather, it could indirectly decrease VA efficacy by counteracting the effect of VA binding or regulate the process disrupted by VAs.	bind
43395	1	10202	5	11	NULL	NULL	NULL				bind			HisRS-related domain		tRNA	NucleicAcid	uncharged			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_22_22820_s_37	15010461	A final proposed role for the extreme carboxyl terminus of Gcn2p is to facilitate binding of the HisRS-related domain to uncharged tRNA ( ).	bind
43396	2	10202	5	11	NULL	NULL	NULL	Gcn2p	GP		facilitates		possibly	carboxyl terminus		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_22_22820_s_37	15010461	A final proposed role for the extreme carboxyl terminus of Gcn2p is to facilitate binding of the HisRS-related domain to uncharged tRNA ( ).	bind
36361	1	10202	6	NULL	NULL	0	NULL		NULL		bind	NULL		HisRS-related domain		tRNA	NULL	uncharged			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_22_22820_s_37	15010461	A final proposed role for the extreme carboxyl terminus of Gcn2p is to facilitate binding of the HisRS-related domain to uncharged tRNA ( ).	bind
36362	2	10202	6	10	NULL	0	NULL	Gcn2p			facilitate		possibly	carboxyl terminus		statement 1					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_22_22820_s_37	15010461	A final proposed role for the extreme carboxyl terminus of Gcn2p is to facilitate binding of the HisRS-related domain to uncharged tRNA ( ).	bind
43397	1	10203	5	NULL	NULL	0	NULL	SAP97	NULL		is important for	NULL		GK domain		presynaptic effects	NULL	transducing			NULL		0	NULL	NULL	NULL	gw70_jneurosci_26_8_2343_s_358	16495462	A final region of SAP97 found to be important for transducing its presynaptic effects is the GK domain, which binds members of the GK associated protein/SAP90/PSD-95-associated protein (GKAP/SAPAP) family (Kim et al., 1997 ; Takeuchi et al., 1997 ) and SPAR/SPAL, an actin binding protein with RapGAP activity (Pak et al., 2001 ; Roy et al., 2002 ).	bind
43440	2	10203	5	NULL	NULL	0	NULL	SAP97	NULL		bind	NULL		GK domain		GKAP/SAPAP family	NULL	members of			NULL		0	NULL	NULL	NULL	gw70_jneurosci_26_8_2343_s_358	16495462	A final region of SAP97 found to be important for transducing its presynaptic effects is the GK domain, which binds members of the GK associated protein/SAP90/PSD-95-associated protein (GKAP/SAPAP) family (Kim et al., 1997 ; Takeuchi et al., 1997 ) and SPAR/SPAL, an actin binding protein with RapGAP activity (Pak et al., 2001 ; Roy et al., 2002 ).	bind
43441	3	10203	5	NULL	NULL	0	NULL	GKAP/SAPAP family	NULL		is	NULL				GK associated protein/SAP90/PSD-95-associated protein family	NULL				NULL		0	NULL	NULL	NULL	gw70_jneurosci_26_8_2343_s_358	16495462	A final region of SAP97 found to be important for transducing its presynaptic effects is the GK domain, which binds members of the GK associated protein/SAP90/PSD-95-associated protein (GKAP/SAPAP) family (Kim et al., 1997 ; Takeuchi et al., 1997 ) and SPAR/SPAL, an actin binding protein with RapGAP activity (Pak et al., 2001 ; Roy et al., 2002 ).	bind
43442	4	10203	5	NULL	NULL	0	NULL	SPAR/SPAL	NULL		is a type of	NULL				actin binding protein	NULL				NULL		0	NULL	NULL	NULL	gw70_jneurosci_26_8_2343_s_358	16495462	A final region of SAP97 found to be important for transducing its presynaptic effects is the GK domain, which binds members of the GK associated protein/SAP90/PSD-95-associated protein (GKAP/SAPAP) family (Kim et al., 1997 ; Takeuchi et al., 1997 ) and SPAR/SPAL, an actin binding protein with RapGAP activity (Pak et al., 2001 ; Roy et al., 2002 ).	bind
43443	5	10203	5	10	NULL	0	NULL	SPAR/SPAL			contains					RapGAP activity					NULL		NULL	NULL	NULL	NULL	gw70_jneurosci_26_8_2343_s_358	16495462	A final region of SAP97 found to be important for transducing its presynaptic effects is the GK domain, which binds members of the GK associated protein/SAP90/PSD-95-associated protein (GKAP/SAPAP) family (Kim et al., 1997 ; Takeuchi et al., 1997 ) and SPAR/SPAL, an actin binding protein with RapGAP activity (Pak et al., 2001 ; Roy et al., 2002 ).	bind
43444	6	10203	5	NULL	NULL	0	NULL	SAP97	NULL		bind	NULL		GK domain		SPAR/SPAL	NULL				NULL		0	NULL	NULL	NULL	gw70_jneurosci_26_8_2343_s_358	16495462	A final region of SAP97 found to be important for transducing its presynaptic effects is the GK domain, which binds members of the GK associated protein/SAP90/PSD-95-associated protein (GKAP/SAPAP) family (Kim et al., 1997 ; Takeuchi et al., 1997 ) and SPAR/SPAL, an actin binding protein with RapGAP activity (Pak et al., 2001 ; Roy et al., 2002 ).	bind
36428	1	10203	6	NULL	NULL	0	NULL	SAP97	NULL		bind	NULL		GK domain		GKAP/SAPAP family	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jneurosci_26_8_2343_s_358	16495462	A final region of SAP97 found to be important for transducing its presynaptic effects is the GK domain, which binds members of the GK associated protein/SAP90/PSD-95-associated protein (GKAP/SAPAP) family (Kim et al., 1997 ; Takeuchi et al., 1997 ) and SPAR/SPAL, an actin binding protein with RapGAP activity (Pak et al., 2001 ; Roy et al., 2002 ).	bind
36429	2	10203	6	10	NULL	0	NULL	GKAP/SAPAP family			is					GK associated protein/SAP90/PSD-95-associated protein family					NULL		NULL	NULL	NULL	NULL	gw70_jneurosci_26_8_2343_s_358	16495462	A final region of SAP97 found to be important for transducing its presynaptic effects is the GK domain, which binds members of the GK associated protein/SAP90/PSD-95-associated protein (GKAP/SAPAP) family (Kim et al., 1997 ; Takeuchi et al., 1997 ) and SPAR/SPAL, an actin binding protein with RapGAP activity (Pak et al., 2001 ; Roy et al., 2002 ).	bind
36431	4	10203	6	NULL	NULL	0	NULL	SAP97	NULL		bind	NULL		GK domain		SPAR/SPAL	NULL				NULL		0	NULL	NULL	NULL	gw70_jneurosci_26_8_2343_s_358	16495462	A final region of SAP97 found to be important for transducing its presynaptic effects is the GK domain, which binds members of the GK associated protein/SAP90/PSD-95-associated protein (GKAP/SAPAP) family (Kim et al., 1997 ; Takeuchi et al., 1997 ) and SPAR/SPAL, an actin binding protein with RapGAP activity (Pak et al., 2001 ; Roy et al., 2002 ).	bind
36433	5	10203	6	NULL	NULL	0	NULL	SPAR/SPAL	NULL		is a type of	NULL				actin binding protein	NULL				NULL		0	NULL	NULL	NULL	gw70_jneurosci_26_8_2343_s_358	16495462	A final region of SAP97 found to be important for transducing its presynaptic effects is the GK domain, which binds members of the GK associated protein/SAP90/PSD-95-associated protein (GKAP/SAPAP) family (Kim et al., 1997 ; Takeuchi et al., 1997 ) and SPAR/SPAL, an actin binding protein with RapGAP activity (Pak et al., 2001 ; Roy et al., 2002 ).	bind
36434	6	10203	6	10	NULL	0	NULL	SPAR/SPAL			contains					RapGAP activity					NULL		NULL	NULL	NULL	NULL	gw70_jneurosci_26_8_2343_s_358	16495462	A final region of SAP97 found to be important for transducing its presynaptic effects is the GK domain, which binds members of the GK associated protein/SAP90/PSD-95-associated protein (GKAP/SAPAP) family (Kim et al., 1997 ; Takeuchi et al., 1997 ) and SPAR/SPAL, an actin binding protein with RapGAP activity (Pak et al., 2001 ; Roy et al., 2002 ).	bind
36435	3	10203	6	10	NULL	0	NULL	SAP97			is important for			GK domain		presynaptic effects		transducing			NULL		NULL	NULL	NULL	NULL	gw70_jneurosci_26_8_2343_s_358	16495462	A final region of SAP97 found to be important for transducing its presynaptic effects is the GK domain, which binds members of the GK associated protein/SAP90/PSD-95-associated protein (GKAP/SAPAP) family (Kim et al., 1997 ; Takeuchi et al., 1997 ) and SPAR/SPAL, an actin binding protein with RapGAP activity (Pak et al., 2001 ; Roy et al., 2002 ).	bind
43445	1	10204	5	11	NULL	NULL	NULL	enzymes	GP	mutant	bind					TP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_13_11289_s_471	12522214	A final support for the interpretation that mutant enzymes bind TP in a nonproductive mode is obtained by examination of the catalytic competence of the enzyme-TP covalent complexes of individual mutant enzymes.	bind
36387	1	10204	6	NULL	NULL	0	NULL	enzymes	NULL	mutant	bind	NULL				TP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_13_11289_s_471	12522214	A final support for the interpretation that mutant enzymes bind TP in a nonproductive mode is obtained by examination of the catalytic competence of the enzyme-TP covalent complexes of individual mutant enzymes.	bind
43447	1	10206	5	11	NULL	NULL	NULL	LexA	GP	E. coli	bind		differentially							SOS box	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_8_2201_s_316	9555905	A finding of an equal affinity of DinR for each DinR box would contrast dramatically with the finding that  E. coli uses differential binding of LexA to its SOS box to regulate damage-inducible gene expression.	bind
43448	2	10206	5	11	NULL	NULL	NULL	statement 1	GP		regulates					damage-inducible gene	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_8_2201_s_316	9555905	A finding of an equal affinity of DinR for each DinR box would contrast dramatically with the finding that  E. coli uses differential binding of LexA to its SOS box to regulate damage-inducible gene expression.	bind
43449	3	10206	5	11	NULL	NULL	NULL	DinR	GP		affinity to									DinR box	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_8_2201_s_316	9555905	A finding of an equal affinity of DinR for each DinR box would contrast dramatically with the finding that  E. coli uses differential binding of LexA to its SOS box to regulate damage-inducible gene expression.	bind
36388	1	10206	6	NULL	NULL	0	NULL	LexA	NULL	E.coli	bind	NULL	differentially				NULL			SOS box	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_8_2201_s_316	9555905	A finding of an equal affinity of DinR for each DinR box would contrast dramatically with the finding that  E. coli uses differential binding of LexA to its SOS box to regulate damage-inducible gene expression.	bind
36389	2	10206	6	10	NULL	0	NULL	statement 1	NULL		regulates	NULL				damage-inducible gene	NULL	expression of			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_8_2201_s_316	9555905	A finding of an equal affinity of DinR for each DinR box would contrast dramatically with the finding that  E. coli uses differential binding of LexA to its SOS box to regulate damage-inducible gene expression.	bind
36390	3	10206	6	NULL	NULL	0	NULL	DinR	NULL		has affinity for	NULL					NULL			DinR box	NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_8_2201_s_316	9555905	A finding of an equal affinity of DinR for each DinR box would contrast dramatically with the finding that  E. coli uses differential binding of LexA to its SOS box to regulate damage-inducible gene expression.	bind
43453	1	10207	5	11	NULL	NULL	NULL	AHR	GP		bind									DREs	NULL		NULL	NULL	NULL	NULL	gw60_annurevcelldevbiol_12_0_55_s_116	8970722	A finding with great impact on how we think of AHR signaling was  the determination that the AHR bound to DREs as part of a  heterodimeric complex ( Elferink et al 1990,  Reyes et al 1992,  Dolwick et al 1993b).	bind
43454	2	10207	5	11	NULL	NULL	NULL	statement 1	GP		is a part of					heterodimeric complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_annurevcelldevbiol_12_0_55_s_116	8970722	A finding with great impact on how we think of AHR signaling was  the determination that the AHR bound to DREs as part of a  heterodimeric complex ( Elferink et al 1990,  Reyes et al 1992,  Dolwick et al 1993b).	bind
36391	1	10207	6	NULL	NULL	0	NULL	AHR 	NULL		is part of the	NULL				heterodimeric complex	NULL				NULL		NULL	NULL	NULL	NULL	gw60_annurevcelldevbiol_12_0_55_s_116	8970722	A finding with great impact on how we think of AHR signaling was  the determination that the AHR bound to DREs as part of a  heterodimeric complex ( Elferink et al 1990,  Reyes et al 1992,  Dolwick et al 1993b).	bind
36392	2	10207	6	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL					NULL			DRE	NULL		0	NULL	NULL	NULL	gw60_annurevcelldevbiol_12_0_55_s_116	8970722	A finding with great impact on how we think of AHR signaling was  the determination that the AHR bound to DREs as part of a  heterodimeric complex ( Elferink et al 1990,  Reyes et al 1992,  Dolwick et al 1993b).	bind
43455	1	10209	5	11	NULL	NULL	NULL	finger protein	GP		similar to		structurally			TFIIIA	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_1_58_s_493	11782445	A finger protein structurally similar to TFIIIA that binds exclusively to 5S RNA in  Xenopus.	bind
43456	2	10209	5	11	NULL	NULL	NULL	statement 1	GP		bind		exclusively			5S RNA	NucleicAcid	Xenopus			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_1_58_s_493	11782445	A finger protein structurally similar to TFIIIA that binds exclusively to 5S RNA in  Xenopus.	bind
36393	1	10209	6	10	NULL	0	NULL	finger protein	NULL		is similar to	NULL	structurally			TFIIIA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_1_58_s_493	11782445	A finger protein structurally similar to TFIIIA that binds exclusively to 5S RNA in  Xenopus.	bind
36394	2	10209	6	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL	exclusively			5S RNA	NULL	Xenopus			NULL		0	NULL	NULL	NULL	gw60_genesdev_16_1_58_s_493	11782445	A finger protein structurally similar to TFIIIA that binds exclusively to 5S RNA in  Xenopus.	bind
43457	1	10210	5	11	NULL	NULL	NULL	Nck	GP		bind					TCR-CD3	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_109_7_901_s_186	12110186	A first approach to investigate whether Nck binding to TCR-CD3 plays an important role in TCR-CD3 signaling was to study the activation potency of Nck-CD3  interaction-inducing (OKT3) and noninducing (JOVI.1) antibodies described above     (Figure 5C).	bind
36395	1	10210	6	NULL	NULL	0	NULL	Nck	NULL		bind	NULL				TCR-CD3	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_109_7_901_s_186	12110186	A first approach to investigate whether Nck binding to TCR-CD3 plays an important role in TCR-CD3 signaling was to study the activation potency of Nck-CD3  interaction-inducing (OKT3) and noninducing (JOVI.1) antibodies described above     (Figure 5C).	bind
43458	1	10211	5	11	NULL	NULL	NULL	Sm proteins	GP	canonical 	bind					U1 snRNAs	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_12_3451_s_157	10369684	A first complex contains the canonical Sm proteins which bind to the U1, U2, U4 and U5 snRNAs.	bind
43460	2	10211	5	11	NULL	NULL	NULL	Sm proteins	GP	canonical 	bind					U2 snRNAs	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_12_3451_s_157	10369684	A first complex contains the canonical Sm proteins which bind to the U1, U2, U4 and U5 snRNAs.	bind
43461	3	10211	5	11	NULL	NULL	NULL	Sm proteins	GP	canonical 	bind					U4 snRNAs	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_12_3451_s_157	10369684	A first complex contains the canonical Sm proteins which bind to the U1, U2, U4 and U5 snRNAs.	bind
43463	4	10211	5	11	NULL	NULL	NULL	Sm proteins	GP	canonical 	bind					U5 snRNAs	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_12_3451_s_157	10369684	A first complex contains the canonical Sm proteins which bind to the U1, U2, U4 and U5 snRNAs.	bind
36396	1	10211	6	10	NULL	0	NULL	Sm proteins	NULL	canonical 	bind	NULL				U1 snRNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_12_3451_s_157	10369684	A first complex contains the canonical Sm proteins which bind to the U1, U2, U4 and U5 snRNAs.	bind
36397	2	10211	6	10	NULL	0	NULL	Sm proteins	NULL	canonical 	bind	NULL				U2 snRNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_12_3451_s_157	10369684	A first complex contains the canonical Sm proteins which bind to the U1, U2, U4 and U5 snRNAs.	bind
36398	3	10211	6	10	NULL	0	NULL	Sm proteins	NULL	canonical 	bind	NULL				U4 snRNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_12_3451_s_157	10369684	A first complex contains the canonical Sm proteins which bind to the U1, U2, U4 and U5 snRNAs.	bind
36399	4	10211	6	10	NULL	0	NULL	Sm proteins	NULL	canonical 	bind	NULL				U5 snRNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_12_3451_s_157	10369684	A first complex contains the canonical Sm proteins which bind to the U1, U2, U4 and U5 snRNAs.	bind
43464	1	10213	5	11	NULL	NULL	NULL	single-chain flavohemoglobins	GP		consists of								C-terminal FAD binding domain		NULL		NULL	NULL	NULL	NULL	gw60_embo_19_11_2424_s_12	10835341	A first group, occurring in bacteria and fungi, includes single-chain flavohemoglobins, which consist of an N-terminal heme-containing domain displaying a conventional globin fold, and a C-terminal FAD or NADP+ binding domain structurally related to ferredoxin NADP+ reductase ( Ermler  et al., 1995).	bind
43465	2	10213	5	11	NULL	NULL	NULL	single-chain flavohemoglobins	GP		consists of								C-terminal FAD binding domain		NULL		NULL	NULL	NULL	NULL	gw60_embo_19_11_2424_s_12	10835341	A first group, occurring in bacteria and fungi, includes single-chain flavohemoglobins, which consist of an N-terminal heme-containing domain displaying a conventional globin fold, and a C-terminal FAD or NADP+ binding domain structurally related to ferredoxin NADP+ reductase ( Ermler  et al., 1995).	bind
43467	3	10213	5	11	NULL	NULL	NULL	single-chain flavohemoglobins	GP		displays			N-terminal heme-containing domain 		globin fold	GP	conventional 			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_11_2424_s_12	10835341	A first group, occurring in bacteria and fungi, includes single-chain flavohemoglobins, which consist of an N-terminal heme-containing domain displaying a conventional globin fold, and a C-terminal FAD or NADP+ binding domain structurally related to ferredoxin NADP+ reductase ( Ermler  et al., 1995).	bind
43468	4	10213	5	11	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_11_2424_s_12	10835341	A first group, occurring in bacteria and fungi, includes single-chain flavohemoglobins, which consist of an N-terminal heme-containing domain displaying a conventional globin fold, and a C-terminal FAD or NADP+ binding domain structurally related to ferredoxin NADP+ reductase ( Ermler  et al., 1995).	bind
43469	5	10213	5	11	NULL	NULL	NULL	statement 4	Process		is related to		structurally			ferredoxin NADP+ reductase	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_11_2424_s_12	10835341	A first group, occurring in bacteria and fungi, includes single-chain flavohemoglobins, which consist of an N-terminal heme-containing domain displaying a conventional globin fold, and a C-terminal FAD or NADP+ binding domain structurally related to ferredoxin NADP+ reductase ( Ermler  et al., 1995).	bind
36437	1	10213	6	10	NULL	0	NULL	single-chain flavohemoglobins			displays a			N-terminal heme-containing domain		globin fold		conventional			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_11_2424_s_12	10835341	A first group, occurring in bacteria and fungi, includes single-chain flavohemoglobins, which consist of an N-terminal heme-containing domain displaying a conventional globin fold, and a C-terminal FAD or NADP+ binding domain structurally related to ferredoxin NADP+ reductase ( Ermler  et al., 1995).	bind
36438	2	10213	6	10	NULL	0	NULL	single-chain flavohemoglobins			consists of								C-terminal FAD binding domain		NULL		NULL	NULL	NULL	NULL	gw60_embo_19_11_2424_s_12	10835341	A first group, occurring in bacteria and fungi, includes single-chain flavohemoglobins, which consist of an N-terminal heme-containing domain displaying a conventional globin fold, and a C-terminal FAD or NADP+ binding domain structurally related to ferredoxin NADP+ reductase ( Ermler  et al., 1995).	bind
36439	3	10213	6	10	NULL	0	NULL	single-chain flavohemoglobins			consists of								NADP+ binding domain		NULL		NULL	NULL	NULL	NULL	gw60_embo_19_11_2424_s_12	10835341	A first group, occurring in bacteria and fungi, includes single-chain flavohemoglobins, which consist of an N-terminal heme-containing domain displaying a conventional globin fold, and a C-terminal FAD or NADP+ binding domain structurally related to ferredoxin NADP+ reductase ( Ermler  et al., 1995).	bind
36440	4	10213	6	10	NULL	0	NULL	statement 2			is an alternative to					statement 3					NULL		NULL	NULL	NULL	NULL	gw60_embo_19_11_2424_s_12	10835341	A first group, occurring in bacteria and fungi, includes single-chain flavohemoglobins, which consist of an N-terminal heme-containing domain displaying a conventional globin fold, and a C-terminal FAD or NADP+ binding domain structurally related to ferredoxin NADP+ reductase ( Ermler  et al., 1995).	bind
57484	5	10213	6	10	NULL	0	NULL	statement 4			is related to		structurally			ferredoxin NADP+ reductase					NULL		NULL	NULL	NULL	NULL	gw60_embo_19_11_2424_s_12	10835341	A first group, occurring in bacteria and fungi, includes single-chain flavohemoglobins, which consist of an N-terminal heme-containing domain displaying a conventional globin fold, and a C-terminal FAD or NADP+ binding domain structurally related to ferredoxin NADP+ reductase ( Ermler  et al., 1995).	bind
43470	1	10214	5	11	NULL	NULL	NULL	citrate synthase	GP	heat-denatured	bind					Hsp25	GP	mammalian			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_18_11032_s_166	9556585	A first indication that sHsps may collaborate with other chaperones in the refolding of bound denatured proteins came from the observation that the refolding of heat-denatured citrate synthase bound to mammalian Hsp25, can be activated by Hsp70, even without ATP ( 4).	bind
43471	2	10214	5	11	NULL	NULL	NULL	Hsp70	GP		activates					statement 1	Process	refolding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_18_11032_s_166	9556585	A first indication that sHsps may collaborate with other chaperones in the refolding of bound denatured proteins came from the observation that the refolding of heat-denatured citrate synthase bound to mammalian Hsp25, can be activated by Hsp70, even without ATP ( 4).	bind
43472	3	10214	5	11	NULL	NULL	NULL	ATP	Chemical		is not required for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_18_11032_s_166	9556585	A first indication that sHsps may collaborate with other chaperones in the refolding of bound denatured proteins came from the observation that the refolding of heat-denatured citrate synthase bound to mammalian Hsp25, can be activated by Hsp70, even without ATP ( 4).	bind
43475	6	10214	5	11	NULL	NULL	NULL	statement 4	Process		leads to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_18_11032_s_166	9556585	A first indication that sHsps may collaborate with other chaperones in the refolding of bound denatured proteins came from the observation that the refolding of heat-denatured citrate synthase bound to mammalian Hsp25, can be activated by Hsp70, even without ATP ( 4).	bind
36400	1	10214	6	NULL	NULL	0	NULL	citrate synthase	NULL	heat denatured	bind	NULL				Hsp25	NULL	mammalian			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_18_11032_s_166	9556585	A first indication that sHsps may collaborate with other chaperones in the refolding of bound denatured proteins came from the observation that the refolding of heat-denatured citrate synthase bound to mammalian Hsp25, can be activated by Hsp70, even without ATP ( 4).	bind
36401	2	10214	6	10	NULL	0	NULL	Hsp70			activates					statement 1		refolding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_18_11032_s_166	9556585	A first indication that sHsps may collaborate with other chaperones in the refolding of bound denatured proteins came from the observation that the refolding of heat-denatured citrate synthase bound to mammalian Hsp25, can be activated by Hsp70, even without ATP ( 4).	bind
36402	3	10214	6	NULL	NULL	0	NULL	statement 2	NULL		occurs without	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_18_11032_s_166	9556585	A first indication that sHsps may collaborate with other chaperones in the refolding of bound denatured proteins came from the observation that the refolding of heat-denatured citrate synthase bound to mammalian Hsp25, can be activated by Hsp70, even without ATP ( 4).	bind
43476	1	10215	5	11	NULL	NULL	NULL	Hsp40	GP		bind					unfolded proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_51_36757_s_226	10593983	A first possibility is that binding of Hsp40 to unfolded proteins is essential for their delivery to Hsp70 and that this capacity is lost in the Hsp40 mutants.	bind
43477	2	10215	5	11	NULL	NULL	NULL	unfolded proteins	GP		are delivered to					Hsp70	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_51_36757_s_226	10593983	A first possibility is that binding of Hsp40 to unfolded proteins is essential for their delivery to Hsp70 and that this capacity is lost in the Hsp40 mutants.	bind
43478	3	10215	5	11	NULL	NULL	NULL	statement 1	Process		is essential for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_51_36757_s_226	10593983	A first possibility is that binding of Hsp40 to unfolded proteins is essential for their delivery to Hsp70 and that this capacity is lost in the Hsp40 mutants.	bind
43479	4	10215	5	11	NULL	NULL	NULL	Hsp40	GP	mutant	does not bind					unfolded proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_51_36757_s_226	10593983	A first possibility is that binding of Hsp40 to unfolded proteins is essential for their delivery to Hsp70 and that this capacity is lost in the Hsp40 mutants.	bind
36403	1	10215	6	NULL	NULL	0	NULL	Hsp40	NULL		bind	NULL				unfolded proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_51_36757_s_226	10593983	A first possibility is that binding of Hsp40 to unfolded proteins is essential for their delivery to Hsp70 and that this capacity is lost in the Hsp40 mutants.	bind
36441	2	10215	6	NULL	NULL	0	NULL	unfolded proteins	NULL		are delivered to	NULL				Hsp70	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_51_36757_s_226	10593983	A first possibility is that binding of Hsp40 to unfolded proteins is essential for their delivery to Hsp70 and that this capacity is lost in the Hsp40 mutants.	bind
36442	3	10215	6	NULL	NULL	0	NULL	statement 1	NULL		is essential for	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_51_36757_s_226	10593983	A first possibility is that binding of Hsp40 to unfolded proteins is essential for their delivery to Hsp70 and that this capacity is lost in the Hsp40 mutants.	bind
36443	4	10215	6	NULL	NULL	0	NULL	Hsp40	NULL	mutant	does not bind	NULL				unfolded proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_51_36757_s_226	10593983	A first possibility is that binding of Hsp40 to unfolded proteins is essential for their delivery to Hsp70 and that this capacity is lost in the Hsp40 mutants.	bind
43481	1	10217	5	11	NULL	NULL	NULL	Mad2	GP		bind					Cdc20	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_10_4584_s_28	15269280	A first series of studies showed that Mad2 binds to Cdc20 and thereby inhibits APC/Cdc20 ubiquitination activity (Li  et al., 1997 ; Fang  et al., 1998 ; Hwang  et al., 1998 ; Kim  et al., 1998 ).	bind
43482	2	10217	5	11	NULL	NULL	NULL	statement 1	Process		inhibits					APC/Cdc20	GP	ubiquitination of			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_10_4584_s_28	15269280	A first series of studies showed that Mad2 binds to Cdc20 and thereby inhibits APC/Cdc20 ubiquitination activity (Li  et al., 1997 ; Fang  et al., 1998 ; Hwang  et al., 1998 ; Kim  et al., 1998 ).	bind
36404	1	10217	6	NULL	NULL	0	NULL	Mad2	NULL		bind	NULL				Cdc20	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_10_4584_s_28	15269280	A first series of studies showed that Mad2 binds to Cdc20 and thereby inhibits APC/Cdc20 ubiquitination activity (Li  et al., 1997 ; Fang  et al., 1998 ; Hwang  et al., 1998 ; Kim  et al., 1998 ).	bind
36405	2	10217	6	NULL	NULL	0	NULL	statement 1	NULL		inhibits	NULL				APC/Cdc20	NULL	ubiquitination of			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_10_4584_s_28	15269280	A first series of studies showed that Mad2 binds to Cdc20 and thereby inhibits APC/Cdc20 ubiquitination activity (Li  et al., 1997 ; Fang  et al., 1998 ; Hwang  et al., 1998 ; Kim  et al., 1998 ).	bind
43483	1	10218	5	NULL	NULL	0	NULL	Cre	NULL		mediate	NULL				DNA recombination	NULL	site-specific			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_13_2764_s_2	12087159	A first step in Cre-mediated site-specific DNA recombination is binding to the two 13 bp repeats of the 34 bp site  loxP.	bind
48408	2	10218	5	10	NULL	0	NULL	Cre	NULL		bind	NULL				loxP	NULL			13 bp repeats of the 34 bp site 	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_13_2764_s_2	12087159	A first step in Cre-mediated site-specific DNA recombination is binding to the two 13 bp repeats of the 34 bp site  loxP.	bind
36406	1	10218	6	10	NULL	0	NULL	Cre	NULL		mediates	NULL				DNA recombination	NULL	site-specific			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_13_2764_s_2	12087159	A first step in Cre-mediated site-specific DNA recombination is binding to the two 13 bp repeats of the 34 bp site  loxP.	bind
48409	2	10218	6	10	NULL	0	NULL	Cre	NULL		bind	NULL				loxP	NULL			13 bp repeats of the 34 bp site	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_13_2764_s_2	12087159	A first step in Cre-mediated site-specific DNA recombination is binding to the two 13 bp repeats of the 34 bp site  loxP.	bind
43487	1	10219	5	11	NULL	NULL	NULL	top1	GP	reconstituted;;human	lacks							whole	linker domain		NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_9_871_s_216	11564555	A first work on reconstituted human top1 showed that the lack of the whole linker domain decreased DNA binding and cleavage levels with CPT  [34]  .	bind
43488	2	10219	5	11	NULL	NULL	NULL	statement 1	Process		decrease					DNA	NucleicAcid	binding of			NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_9_871_s_216	11564555	A first work on reconstituted human top1 showed that the lack of the whole linker domain decreased DNA binding and cleavage levels with CPT  [34]  .	bind
43489	3	10219	5	11	NULL	NULL	NULL	statement 1	Process		decrease					CPT	Chemical	cleavage levels with			NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_9_871_s_216	11564555	A first work on reconstituted human top1 showed that the lack of the whole linker domain decreased DNA binding and cleavage levels with CPT  [34]  .	bind
36444	1	10219	6	NULL	NULL	0	NULL	top1	NULL	human	bind	NULL		linker domain		DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_chembiol_8_9_871_s_216	11564555	A first work on reconstituted human top1 showed that the lack of the whole linker domain decreased DNA binding and cleavage levels with CPT  [34]  .	bind
36445	2	10219	6	NULL	NULL	0	NULL	top1	NULL	human;; lack of	decreases 	NULL		linker domain		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_chembiol_8_9_871_s_216	11564555	A first work on reconstituted human top1 showed that the lack of the whole linker domain decreased DNA binding and cleavage levels with CPT  [34]  .	bind
36446	3	10219	6	NULL	NULL	0	NULL	top1	NULL	human;; lack of	decreases	NULL		linker domain		CPT	NULL	clevage levels with			NULL		0	NULL	NULL	NULL	gw60_chembiol_8_9_871_s_216	11564555	A first work on reconstituted human top1 showed that the lack of the whole linker domain decreased DNA binding and cleavage levels with CPT  [34]  .	bind
43490	1	10220	5	11	NULL	NULL	NULL	F-actin	GP		bind		weakly			vimentin	GP		tail domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_41_30393_s_126	16901892	A fit of the binding curve using nonlinear regression (supplemental Fig. S1) yielded an equilibrium dissociation constant,  kd, of  13.8 muM, indicative of weak binding between F-actin and the tail domain of vimentin.	bind
36407	1	10220	6	NULL	NULL	0	NULL	F-actin	NULL		bind	NULL	weakly			vimentin	NULL		tail domain		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_41_30393_s_126	16901892	A fit of the binding curve using nonlinear regression (supplemental Fig. S1) yielded an equilibrium dissociation constant,  kd, of  13.8 muM, indicative of weak binding between F-actin and the tail domain of vimentin.	bind
43491	1	10221	5	NULL	NULL	0	NULL	Ffh	NULL		bind	NULL				FtsY	NULL				NULL		0	NULL	NULL	NULL	gw60_science_288_5471_1640_s_49	10834842	A fit of the data to the equation  kobs =  kon[protein] +  koff gave values of  kon = 5.6 ( plus-or-minus 0.6) x 102 M 1 s 1 and 9.2 ( plus-or-minus 0.7) x 104 M 1 s 1 for the binding of Ffh and the Ffh/4.5 S RNP, respectively, to FtsY.	bind
43492	2	10221	5	NULL	NULL	0	NULL	Ffh/4.5 S RNP	NULL		bind	NULL				FtsY	NULL				NULL		0	NULL	NULL	NULL	gw60_science_288_5471_1640_s_49	10834842	A fit of the data to the equation  kobs =  kon[protein] +  koff gave values of  kon = 5.6 ( plus-or-minus 0.6) x 102 M 1 s 1 and 9.2 ( plus-or-minus 0.7) x 104 M 1 s 1 for the binding of Ffh and the Ffh/4.5 S RNP, respectively, to FtsY.	bind
36408	1	10221	6	NULL	NULL	0	NULL	Ffh	NULL		bind	NULL				FtsY	NULL				NULL		0	NULL	NULL	NULL	gw60_science_288_5471_1640_s_49	10834842	A fit of the data to the equation  kobs =  kon[protein] +  koff gave values of  kon = 5.6 ( plus-or-minus 0.6) x 102 M 1 s 1 and 9.2 ( plus-or-minus 0.7) x 104 M 1 s 1 for the binding of Ffh and the Ffh/4.5 S RNP, respectively, to FtsY.	bind
36409	2	10221	6	NULL	NULL	0	NULL	Ffh/4.5 S RNP	NULL		bind	NULL				FtsY	NULL				NULL		0	NULL	NULL	NULL	gw60_science_288_5471_1640_s_49	10834842	A fit of the data to the equation  kobs =  kon[protein] +  koff gave values of  kon = 5.6 ( plus-or-minus 0.6) x 102 M 1 s 1 and 9.2 ( plus-or-minus 0.7) x 104 M 1 s 1 for the binding of Ffh and the Ffh/4.5 S RNP, respectively, to FtsY.	bind
43493	1	10222	5	11	NULL	NULL	NULL	sV(HIgR)-Fc	GP		bind		saturable			gD	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_26_15700_s_175	9861033	A fixed amount of sV(HIgR)-Fc (10 nM), giving saturable binding to gD in  A, was mixed with increasing amounts of IgGs from the indicated antibodies and then allowed to react with gD, preimmobilized to microwells.	bind
48549	1	10222	6	NULL	NULL	0	NULL	sV(HIgR)-Fc	NULL		bind	NULL				gD	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_26_15700_s_175	9861033	A fixed amount of sV(HIgR)-Fc (10 nM), giving saturable binding to gD in  A, was mixed with increasing amounts of IgGs from the indicated antibodies and then allowed to react with gD, preimmobilized to microwells.	bind
43494	1	10223	5	11	NULL	NULL	NULL	Mant-ATP 	Chemical		bind					CDK2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_13_8746_s_248	10085115	A fixed concentration of CDK2 (0.2 muM) ( open symbols) and phosphorylated CDK2 ( closed symbols) were titrated with increasing concentrations of ATP ( ,  ) and ADP (  , ).  b, Mant-ATP and Mant-ADP binding to CDK2 and phosphorylated CDK2.	bind
43497	2	10223	5	11	NULL	NULL	NULL	Mant-ADP	Chemical		bind					CDK2	GP	phosphorylated			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_13_8746_s_248	10085115	A fixed concentration of CDK2 (0.2 muM) ( open symbols) and phosphorylated CDK2 ( closed symbols) were titrated with increasing concentrations of ATP ( ,  ) and ADP (  , ).  b, Mant-ATP and Mant-ADP binding to CDK2 and phosphorylated CDK2.	bind
36410	1	10223	6	NULL	NULL	0	NULL	Mant-ATP	NULL		bind	NULL				CDK2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_13_8746_s_248	10085115	A fixed concentration of CDK2 (0.2 muM) ( open symbols) and phosphorylated CDK2 ( closed symbols) were titrated with increasing concentrations of ATP ( ,  ) and ADP (  , ).  b, Mant-ATP and Mant-ADP binding to CDK2 and phosphorylated CDK2.	bind
36411	2	10223	6	NULL	NULL	0	NULL	Mant-ADP	NULL		bind	NULL				CDK2	NULL	phosphorylated			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_13_8746_s_248	10085115	A fixed concentration of CDK2 (0.2 muM) ( open symbols) and phosphorylated CDK2 ( closed symbols) were titrated with increasing concentrations of ATP ( ,  ) and ADP (  , ).  b, Mant-ATP and Mant-ADP binding to CDK2 and phosphorylated CDK2.	bind
43553	1	10224	5	11	NULL	NULL	NULL	netrin1 gene	GP	zebrafish	requires				floor plate enhancer	Cyclops	Organism	signaling of			NULL		NULL	NULL	NULL	NULL	gw60_development_130_14_3331_s_465	12783802	A floor plate enhancer of the zebrafish netrin1 gene requires Cyclops (Nodal) signalling and the winged helix transcription factor FoxA2.	bind
43554	2	10224	5	11	NULL	NULL	NULL	netrin1 gene	GP	zebrafish	requires				floor plate enhancer	FoxA2	GP				NULL		NULL	NULL	NULL	NULL	gw60_development_130_14_3331_s_465	12783802	A floor plate enhancer of the zebrafish netrin1 gene requires Cyclops (Nodal) signalling and the winged helix transcription factor FoxA2.	bind
43555	3	10224	5	11	NULL	NULL	NULL	FoxA2	GP		is a type of					winged helix transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_development_130_14_3331_s_465	12783802	A floor plate enhancer of the zebrafish netrin1 gene requires Cyclops (Nodal) signalling and the winged helix transcription factor FoxA2.	bind
36412	1	10224	6	NULL	NULL	0	NULL	netrin1 gene	NULL	zebrafish	requires	NULL			floor plate enhancer	FoxA2	NULL				NULL		0	NULL	NULL	NULL	gw60_development_130_14_3331_s_465	12783802	A floor plate enhancer of the zebrafish netrin1 gene requires Cyclops (Nodal) signalling and the winged helix transcription factor FoxA2.	bind
36413	2	10224	6	NULL	NULL	0	NULL	FoxA2	NULL		is a type of	NULL				winged helix transcription factor	NULL				NULL		NULL	NULL	NULL	NULL	gw60_development_130_14_3331_s_465	12783802	A floor plate enhancer of the zebrafish netrin1 gene requires Cyclops (Nodal) signalling and the winged helix transcription factor FoxA2.	bind
36414	3	10224	6	NULL	NULL	0	NULL	netrin1 gene	NULL	zebrafish	requires	NULL			floor plate enhancer	Cyclops (Nodal)	NULL	signaling of			NULL		0	NULL	NULL	NULL	gw60_development_130_14_3331_s_465	12783802	A floor plate enhancer of the zebrafish netrin1 gene requires Cyclops (Nodal) signalling and the winged helix transcription factor FoxA2.	bind
43498	1	10225	5	11	NULL	NULL	NULL	LPS	Chemical	E. coli	bind					PBMs	Cell	porcine			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_4_1421_s_122	9529062	A flow cytometric assay was developed to monitor LPS binding to porcine PBMs. Density gradient-isolated cells were incubated with FITC-labelled  E. coli LPS in the presence of autologous serum, and binding to PBMs was characterized by flow cytometry.	bind
36415	1	10225	6	10	NULL	0	NULL	LPS	NULL	E.coli	bind	NULL				PBM	NULL	porcine			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_4_1421_s_122	9529062	A flow cytometric assay was developed to monitor LPS binding to porcine PBMs. Density gradient-isolated cells were incubated with FITC-labelled  E. coli LPS in the presence of autologous serum, and binding to PBMs was characterized by flow cytometry.	bind
43558	1	10226	5	11	NULL	NULL	NULL	methotrexate	Chemical	fluorescein	bind					DHFR	GP	reconstituted			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_pnas_96_10_5394_s_5	10318894	A fluorescence assay also is described, based on stoichiometric binding of fluorescein-methotrexate to reconstituted DHFR  in vivo.	bind
36416	1	10226	6	10	NULL	0	NULL	methotrexate	NULL	fluorescein	bind	NULL				DHFR	NULL	reconstituted			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_pnas_96_10_5394_s_5	10318894	A fluorescence assay also is described, based on stoichiometric binding of fluorescein-methotrexate to reconstituted DHFR  in vivo.	bind
43560	1	10227	5	11	NULL	NULL	NULL	synaptotagmin	GP		penetrates into		directly	Ca2+-binding loop 3 of the C2A domain		lipid bilayers	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_49_32966_s_225	9830048	A fluorescence study revealed that Ca2+-binding loop 3 of the C2A domain of synaptotagmin directly penetrates into lipid bilayers, potentially providing movement or force to trigger neuronal exocytosis ( 37).	bind
43561	2	10227	5	11	NULL	NULL	NULL	statement 1	Process		trigger		potentially			neuronal exocytosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_49_32966_s_225	9830048	A fluorescence study revealed that Ca2+-binding loop 3 of the C2A domain of synaptotagmin directly penetrates into lipid bilayers, potentially providing movement or force to trigger neuronal exocytosis ( 37).	bind
36417	1	10227	6	NULL	NULL	0	NULL	synaptotagmin	NULL		penetrates	NULL	directly	Ca2+-binding loop 3 of the C2A domain		lipid bilayers	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_49_32966_s_225	9830048	A fluorescence study revealed that Ca2+-binding loop 3 of the C2A domain of synaptotagmin directly penetrates into lipid bilayers, potentially providing movement or force to trigger neuronal exocytosis ( 37).	bind
36418	2	10227	6	NULL	NULL	0	NULL	statement 1	NULL		triggers	NULL				neuronal exocytosis	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_49_32966_s_225	9830048	A fluorescence study revealed that Ca2+-binding loop 3 of the C2A domain of synaptotagmin directly penetrates into lipid bilayers, potentially providing movement or force to trigger neuronal exocytosis ( 37).	bind
43563	1	10229	5	11	NULL	NULL	NULL	cyclopamine	Chemical	fluorescent derivative of	bind					Smo-expressing cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_21_2743_s_63	12414725	A fluorescent derivative of cyclopamine binds Smo-expressing cells.	bind
36419	1	10229	6	NULL	NULL	0	NULL	cyclopamine	NULL	fluorescent derivative of	bind	NULL				Smo-expressing cells	NULL				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_21_2743_s_63	12414725	A fluorescent derivative of cyclopamine binds Smo-expressing cells.	bind
43565	1	10230	5	11	NULL	NULL	NULL	cyclopamine	Chemical	fluorescent derivative of	bind		specifically			Smo-expressing cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_21_2743_s_54	12414725	A fluorescent derivative of cyclopamine specifically binds Smo-expressing cells	bind
36420	1	10230	6	NULL	NULL	0	NULL	cyclopamine	NULL	fluorescent derivative of	bind	NULL	specifically			Smo-expressing cells	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_16_21_2743_s_54	12414725	A fluorescent derivative of cyclopamine specifically binds Smo-expressing cells	bind
48726	1	10232	5	11	NULL	NULL	NULL	nuclear proteins	GP	unfractionated testis cells	bind									RE region	NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_68_6_2267_s_214	12606375	A footprint was formed over the RE region by the binding of nuclear proteins derived from unfractionated testis cells and from an enriched population of pachytene primary spermatocytes.	bind
48727	2	10232	5	11	NULL	NULL	NULL	nuclear proteins	GP	pachytene primary spermatocytes	bind									RE region	NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_68_6_2267_s_214	12606375	A footprint was formed over the RE region by the binding of nuclear proteins derived from unfractionated testis cells and from an enriched population of pachytene primary spermatocytes.	bind
36449	1	10232	6	NULL	NULL	0	NULL	nuclear proteins	NULL	unfractionated testis cells 	bind	NULL					NULL			RE region	NULL		0	NULL	NULL	NULL	gw70_biolreprod_68_6_2267_s_214	12606375	A footprint was formed over the RE region by the binding of nuclear proteins derived from unfractionated testis cells and from an enriched population of pachytene primary spermatocytes.	bind
36450	2	10232	6	10	NULL	0	NULL	nuclear proteins		pachytene primary spermatocytes	bind									RE region	NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_68_6_2267_s_214	12606375	A footprint was formed over the RE region by the binding of nuclear proteins derived from unfractionated testis cells and from an enriched population of pachytene primary spermatocytes.	bind
43573	1	10233	5	11	NULL	NULL	NULL	ADP	Chemical		bind		weakly			acto-Myo9b	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_47_38957_s_257	16179355	A forced fit to the observed rates gave an approximate estimate of  KAD of 156 muM, indicating that ADP bound weakly to acto-Myo9b (data not shown).	bind
36421	1	10233	6	NULL	NULL	0	NULL	ADP	NULL		bind	NULL	weakly			acto-Myo9b	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_47_38957_s_257	16179355	A forced fit to the observed rates gave an approximate estimate of  KAD of 156 muM, indicating that ADP bound weakly to acto-Myo9b (data not shown).	bind
43574	1	10234	5	11	NULL	NULL	NULL	UNC-13S	GP		does not bind					DAG	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neuron_24_2_335_s_277	10571228	A form of UNC-13S that does not bind DAG shifts the dose-response curve for phorbol-induced hypersensitivity to aldicarb, suggesting that neurons contain a second low-affinity phorbol receptor that regulates acetylcholine release.	bind
43577	3	10234	5	11	NULL	NULL	NULL	neurons	Cell		contains					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_24_2_335_s_277	10571228	A form of UNC-13S that does not bind DAG shifts the dose-response curve for phorbol-induced hypersensitivity to aldicarb, suggesting that neurons contain a second low-affinity phorbol receptor that regulates acetylcholine release.	bind
43578	2	10234	5	11	NULL	NULL	NULL	phorbol receptor	GP	low-affinity	regulates					acetylcholine	Chemical	release of			NULL		NULL	NULL	NULL	NULL	gw60_neuron_24_2_335_s_277	10571228	A form of UNC-13S that does not bind DAG shifts the dose-response curve for phorbol-induced hypersensitivity to aldicarb, suggesting that neurons contain a second low-affinity phorbol receptor that regulates acetylcholine release.	bind
36451	1	10234	6	NULL	NULL	0	NULL	UNC-13S	NULL		does not bind	NULL				DAG	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_24_2_335_s_277	10571228	A form of UNC-13S that does not bind DAG shifts the dose-response curve for phorbol-induced hypersensitivity to aldicarb, suggesting that neurons contain a second low-affinity phorbol receptor that regulates acetylcholine release.	bind
36452	2	10234	6	NULL	NULL	0	NULL	neurons	NULL		contain	NULL				phorbol receptor	NULL	second low affinity			NULL		0	NULL	NULL	NULL	gw60_neuron_24_2_335_s_277	10571228	A form of UNC-13S that does not bind DAG shifts the dose-response curve for phorbol-induced hypersensitivity to aldicarb, suggesting that neurons contain a second low-affinity phorbol receptor that regulates acetylcholine release.	bind
36453	3	10234	6	NULL	NULL	0	NULL	statement 2	NULL		regulates	NULL				acetylcholine	NULL	release of 			NULL		0	NULL	NULL	NULL	gw60_neuron_24_2_335_s_277	10571228	A form of UNC-13S that does not bind DAG shifts the dose-response curve for phorbol-induced hypersensitivity to aldicarb, suggesting that neurons contain a second low-affinity phorbol receptor that regulates acetylcholine release.	bind
43582	1	10236	5	11	NULL	NULL	NULL	Daam1	GP		is a type of					Formin-Homology Protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_843_s_83	11779461	A Formin-Homology (FH) Protein Daam1 that Binds  to Dvl	bind
43583	2	10236	5	11	NULL	NULL	NULL	Daam1	GP		bind					Dvl	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_843_s_83	11779461	A Formin-Homology (FH) Protein Daam1 that Binds  to Dvl	bind
48426	3	10236	5	11	NULL	NULL	NULL	FH	GP		is					Formin-Homology	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_107_7_843_s_83	11779461	A Formin-Homology (FH) Protein Daam1 that Binds  to Dvl	bind
36422	1	10236	6	NULL	NULL	0	NULL	Daam1	NULL		bind	NULL				Dvl	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_107_7_843_s_83	11779461	A Formin-Homology (FH) Protein Daam1 that Binds  to Dvl	bind
36423	2	10236	6	NULL	NULL	0	NULL	Daam1	NULL		is a type of	NULL				FH protein	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_107_7_843_s_83	11779461	A Formin-Homology (FH) Protein Daam1 that Binds  to Dvl	bind
36424	3	10236	6	NULL	NULL	0	NULL	FH	NULL		is	NULL				Formin-Homology	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_107_7_843_s_83	11779461	A Formin-Homology (FH) Protein Daam1 that Binds  to Dvl	bind
43584	1	10237	5	11	NULL	NULL	NULL	FoTFdeltaN	GP		is					FoTF mutant lacking N-terminal half 	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_4_1175_s_114	15657123	A FoTF mutant lacking the N-terminal half of the protein (FoTFdeltaN) did not bind to TSWV RNA ( Fig. 2 C).	bind
43585	2	10237	5	11	NULL	NULL	NULL	FoTFdeltaN	GP		does not bind					TSWV RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_4_1175_s_114	15657123	A FoTF mutant lacking the N-terminal half of the protein (FoTFdeltaN) did not bind to TSWV RNA ( Fig. 2 C).	bind
36425	1	10237	6	NULL	NULL	0	NULL	FoTFdeltaN	NULL		does not bind	NULL				TSWV RNA	NULL				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_4_1175_s_114	15657123	A FoTF mutant lacking the N-terminal half of the protein (FoTFdeltaN) did not bind to TSWV RNA ( Fig. 2 C).	bind
36426	2	10237	6	10	NULL	0	NULL	FoTFdeltaN	NULL		is	NULL				FoTF mutant lacking the N-terminal half	NULL				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_4_1175_s_114	15657123	A FoTF mutant lacking the N-terminal half of the protein (FoTFdeltaN) did not bind to TSWV RNA ( Fig. 2 C).	bind
43586	1	10238	5	11	NULL	NULL	NULL	E1A	GP		bind					Rb-family proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_15_9966_s_7	12119420	A four amino acid E1A deletion that eliminates binding to Rb-family proteins blocked both repression of TNF-alpha-induced transcription and sensitization to apoptosis.	bind
43587	2	10238	5	11	NULL	NULL	NULL	E1A	GP	four amino acid deletion	eliminate					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_15_9966_s_7	12119420	A four amino acid E1A deletion that eliminates binding to Rb-family proteins blocked both repression of TNF-alpha-induced transcription and sensitization to apoptosis.	bind
43588	3	10238	5	11	NULL	NULL	NULL	TNF-alpha	GP		induce					transcription	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_15_9966_s_7	12119420	A four amino acid E1A deletion that eliminates binding to Rb-family proteins blocked both repression of TNF-alpha-induced transcription and sensitization to apoptosis.	bind
43589	4	10238	5	11	NULL	NULL	NULL	statement 2	Process		block					statement 3	Process	repression of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_15_9966_s_7	12119420	A four amino acid E1A deletion that eliminates binding to Rb-family proteins blocked both repression of TNF-alpha-induced transcription and sensitization to apoptosis.	bind
43591	5	10238	5	11	NULL	NULL	NULL	statement 2	Process		block					apoptosis	Process	sensitization to			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_15_9966_s_7	12119420	A four amino acid E1A deletion that eliminates binding to Rb-family proteins blocked both repression of TNF-alpha-induced transcription and sensitization to apoptosis.	bind
36464	1	10238	6	NULL	NULL	0	NULL	E1A	NULL		bind	NULL				Rb-family proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_15_9966_s_7	12119420	A four amino acid E1A deletion that eliminates binding to Rb-family proteins blocked both repression of TNF-alpha-induced transcription and sensitization to apoptosis.	bind
36465	2	10238	6	10	NULL	0	NULL	E1A		four amino acids deletion of	eliminates					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_15_9966_s_7	12119420	A four amino acid E1A deletion that eliminates binding to Rb-family proteins blocked both repression of TNF-alpha-induced transcription and sensitization to apoptosis.	bind
36466	3	10238	6	NULL	NULL	0	NULL	TNF-alpha	NULL		induces	NULL				transcription	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_15_9966_s_7	12119420	A four amino acid E1A deletion that eliminates binding to Rb-family proteins blocked both repression of TNF-alpha-induced transcription and sensitization to apoptosis.	bind
36467	4	10238	6	10	NULL	0	NULL	statement 2			blocks					statement 3		repression of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_15_9966_s_7	12119420	A four amino acid E1A deletion that eliminates binding to Rb-family proteins blocked both repression of TNF-alpha-induced transcription and sensitization to apoptosis.	bind
36468	5	10238	6	10	NULL	0	NULL	statement 2			blocks					apoptosis		sensitization to			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_15_9966_s_7	12119420	A four amino acid E1A deletion that eliminates binding to Rb-family proteins blocked both repression of TNF-alpha-induced transcription and sensitization to apoptosis.	bind
43592	1	10239	5	11	NULL	NULL	NULL	Bmp2C2	GP		is					fourth Bmp2 DNA region	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_development_131_18_4581_s_165	15342482	A fourth  Bmp2 DNA region,  Bmp2C2, was also bound by the A13-DBD peptide; however, 2- to 4-fold higher concentrations of A13-DBD were required to affect its electrophoretic mobility ( Fig. 2C).	bind
43593	2	10239	5	11	NULL	NULL	NULL	Bmp2C2	GP		bind					A13-DBD peptide	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_development_131_18_4581_s_165	15342482	A fourth  Bmp2 DNA region,  Bmp2C2, was also bound by the A13-DBD peptide; however, 2- to 4-fold higher concentrations of A13-DBD were required to affect its electrophoretic mobility ( Fig. 2C).	bind
36469	1	10239	6	NULL	NULL	0	NULL	Bmp2C2	NULL		bind	NULL				A13DBD peptide	NULL				NULL		0	NULL	NULL	NULL	gw70_development_131_18_4581_s_165	15342482	A fourth  Bmp2 DNA region,  Bmp2C2, was also bound by the A13-DBD peptide; however, 2- to 4-fold higher concentrations of A13-DBD were required to affect its electrophoretic mobility ( Fig. 2C).	bind
36470	2	10239	6	NULL	NULL	0	NULL	Bmp2C2	NULL		is	NULL				fourth Bmp2 DNA region	NULL				NULL		0	NULL	NULL	NULL	gw70_development_131_18_4581_s_165	15342482	A fourth  Bmp2 DNA region,  Bmp2C2, was also bound by the A13-DBD peptide; however, 2- to 4-fold higher concentrations of A13-DBD were required to affect its electrophoretic mobility ( Fig. 2C).	bind
43599	1	10241	5	11	NULL	NULL	NULL	GATA-4	GP		is a type of					zinc finger binding proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_100_2_263_s_12	11165483	A fourth family of transcriptional regulators, the zinc finger binding proteins GATA-4, -5 and -6, are expressed very early in the cardiac program.	bind
43600	2	10241	5	11	NULL	NULL	NULL	GATA-4	GP		is a member of					transcriptional regulators family	GP				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_100_2_263_s_12	11165483	A fourth family of transcriptional regulators, the zinc finger binding proteins GATA-4, -5 and -6, are expressed very early in the cardiac program.	bind
43601	3	10241	5	11	NULL	NULL	NULL	GATA-4	GP		is expressed in		very early			cardiac program	MedicalProcedure				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_100_2_263_s_12	11165483	A fourth family of transcriptional regulators, the zinc finger binding proteins GATA-4, -5 and -6, are expressed very early in the cardiac program.	bind
43602	4	10241	5	11	NULL	NULL	NULL	GATA-5	GP		is a type of					zinc finger binding proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_100_2_263_s_12	11165483	A fourth family of transcriptional regulators, the zinc finger binding proteins GATA-4, -5 and -6, are expressed very early in the cardiac program.	bind
43603	5	10241	5	11	NULL	NULL	NULL	GATA-5	GP		is a member of					transcriptional regulators family	GP				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_100_2_263_s_12	11165483	A fourth family of transcriptional regulators, the zinc finger binding proteins GATA-4, -5 and -6, are expressed very early in the cardiac program.	bind
43604	6	10241	5	11	NULL	NULL	NULL	GATA-5	GP		is expressed in		very early			cardiac program	MedicalProcedure				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_100_2_263_s_12	11165483	A fourth family of transcriptional regulators, the zinc finger binding proteins GATA-4, -5 and -6, are expressed very early in the cardiac program.	bind
43605	7	10241	5	11	NULL	NULL	NULL	GATA-6	GP		is a type of					zinc finger binding proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_100_2_263_s_12	11165483	A fourth family of transcriptional regulators, the zinc finger binding proteins GATA-4, -5 and -6, are expressed very early in the cardiac program.	bind
43606	8	10241	5	11	NULL	NULL	NULL	GATA-6	GP		is a member of					transcriptional regulators family	GP				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_100_2_263_s_12	11165483	A fourth family of transcriptional regulators, the zinc finger binding proteins GATA-4, -5 and -6, are expressed very early in the cardiac program.	bind
43607	9	10241	5	11	NULL	NULL	NULL	GATA-6	GP		is expressed in		very early			cardiac program	MedicalProcedure				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_100_2_263_s_12	11165483	A fourth family of transcriptional regulators, the zinc finger binding proteins GATA-4, -5 and -6, are expressed very early in the cardiac program.	bind
36471	1	10241	6	NULL	NULL	0	NULL	GATA-4	NULL		is a type of	NULL				zinc finger binding protein	NULL				NULL		0	NULL	NULL	NULL	gw60_mechdev_100_2_263_s_12	11165483	A fourth family of transcriptional regulators, the zinc finger binding proteins GATA-4, -5 and -6, are expressed very early in the cardiac program.	bind
36472	2	10241	6	NULL	NULL	0	NULL	GATA-5	NULL		is a type of	NULL				zinc finger binding protein	NULL				NULL		0	NULL	NULL	NULL	gw60_mechdev_100_2_263_s_12	11165483	A fourth family of transcriptional regulators, the zinc finger binding proteins GATA-4, -5 and -6, are expressed very early in the cardiac program.	bind
36473	3	10241	6	NULL	NULL	0	NULL	GATA-6	NULL		is a type of	NULL				zinc finger binding protein	NULL				NULL		0	NULL	NULL	NULL	gw60_mechdev_100_2_263_s_12	11165483	A fourth family of transcriptional regulators, the zinc finger binding proteins GATA-4, -5 and -6, are expressed very early in the cardiac program.	bind
36474	4	10241	6	NULL	NULL	0	NULL	GATA-4	NULL		is a type of	NULL				transcriptional regulator	NULL				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_100_2_263_s_12	11165483	A fourth family of transcriptional regulators, the zinc finger binding proteins GATA-4, -5 and -6, are expressed very early in the cardiac program.	bind
36475	5	10241	6	NULL	NULL	0	NULL	GATA-5	NULL		is a type of	NULL				transcriptional regulator	NULL				NULL		0	NULL	NULL	NULL	gw60_mechdev_100_2_263_s_12	11165483	A fourth family of transcriptional regulators, the zinc finger binding proteins GATA-4, -5 and -6, are expressed very early in the cardiac program.	bind
36476	6	10241	6	NULL	NULL	0	NULL	GATA-6	NULL		is a type of	NULL				transcriptional regulator	NULL				NULL		0	NULL	NULL	NULL	gw60_mechdev_100_2_263_s_12	11165483	A fourth family of transcriptional regulators, the zinc finger binding proteins GATA-4, -5 and -6, are expressed very early in the cardiac program.	bind
36477	7	10241	6	10	NULL	0	NULL	GATA-4	NULL		is expressed 	NULL	early			cardiac program	NULL				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_100_2_263_s_12	11165483	A fourth family of transcriptional regulators, the zinc finger binding proteins GATA-4, -5 and -6, are expressed very early in the cardiac program.	bind
36478	8	10241	6	10	NULL	0	NULL	GATA-5	NULL		is expressed	NULL	early			cardiac program	NULL				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_100_2_263_s_12	11165483	A fourth family of transcriptional regulators, the zinc finger binding proteins GATA-4, -5 and -6, are expressed very early in the cardiac program.	bind
36479	9	10241	6	10	NULL	0	NULL	GATA-6	NULL		is expressed	NULL	early			cardiac program	NULL				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_100_2_263_s_12	11165483	A fourth family of transcriptional regulators, the zinc finger binding proteins GATA-4, -5 and -6, are expressed very early in the cardiac program.	bind
43594	1	10242	5	11	NULL	NULL	NULL	CBP	GP		is					CREB binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_6_704_s_259	10189358	A fourth gene encodes a nuclear protein, CREB binding protein (CBP), that can bind to phosphorylated CREB to serve as a cofactor in the regulation of transcription of target genes.	bind
43595	2	10242	5	11	NULL	NULL	NULL	CBP	GP		is a type of					nuclear protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_6_704_s_259	10189358	A fourth gene encodes a nuclear protein, CREB binding protein (CBP), that can bind to phosphorylated CREB to serve as a cofactor in the regulation of transcription of target genes.	bind
43596	3	10242	5	11	NULL	NULL	NULL	CBP	GP		bind					CREB	GP	phosphorylated			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_6_704_s_259	10189358	A fourth gene encodes a nuclear protein, CREB binding protein (CBP), that can bind to phosphorylated CREB to serve as a cofactor in the regulation of transcription of target genes.	bind
43597	4	10242	5	11	NULL	NULL	NULL	statement 3	GP		serve as					cofactor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_6_704_s_259	10189358	A fourth gene encodes a nuclear protein, CREB binding protein (CBP), that can bind to phosphorylated CREB to serve as a cofactor in the regulation of transcription of target genes.	bind
43598	5	10242	5	11	NULL	NULL	NULL	statement 4	Process		during					target genes	GP	regulation of;; transcription of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_6_704_s_259	10189358	A fourth gene encodes a nuclear protein, CREB binding protein (CBP), that can bind to phosphorylated CREB to serve as a cofactor in the regulation of transcription of target genes.	bind
36480	1	10242	6	NULL	NULL	0	NULL	CBP	NULL		is 	NULL				CREB binding protein	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_6_704_s_259	10189358	A fourth gene encodes a nuclear protein, CREB binding protein (CBP), that can bind to phosphorylated CREB to serve as a cofactor in the regulation of transcription of target genes.	bind
36481	2	10242	6	NULL	NULL	0	NULL	CBP	NULL		bind	NULL				CREB	NULL	phosphorylated			NULL		0	NULL	NULL	NULL	gw60_circulationres_84_6_704_s_259	10189358	A fourth gene encodes a nuclear protein, CREB binding protein (CBP), that can bind to phosphorylated CREB to serve as a cofactor in the regulation of transcription of target genes.	bind
36482	3	10242	6	NULL	NULL	0	NULL	CBP	NULL		acts as a cofactor for	NULL				target genes	NULL	regulation of;; transcription of			NULL		0	NULL	NULL	NULL	gw60_circulationres_84_6_704_s_259	10189358	A fourth gene encodes a nuclear protein, CREB binding protein (CBP), that can bind to phosphorylated CREB to serve as a cofactor in the regulation of transcription of target genes.	bind
36483	4	10242	6	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_84_6_704_s_259	10189358	A fourth gene encodes a nuclear protein, CREB binding protein (CBP), that can bind to phosphorylated CREB to serve as a cofactor in the regulation of transcription of target genes.	bind
57485	5	10242	6	10	NULL	0	NULL	CBP			is a type of					nuclear protein					NULL		0	NULL	NULL	NULL	gw60_circulationres_84_6_704_s_259	10189358	A fourth gene encodes a nuclear protein, CREB binding protein (CBP), that can bind to phosphorylated CREB to serve as a cofactor in the regulation of transcription of target genes.	bind
43608	1	10243	5	11	NULL	NULL	NULL	HBO1	GP		is					histone acetyltransferase bound to ORC	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_64_2_435_s_255	10839822	A fourth human MYST protein is HBO1 (histone acetyltransferase bound  to ORC), which was discovered in a two-hybrid screen on the basis of its interaction with the ORC1 subunit of the origin recognition complex (ORC) ( ).	bind
43609	2	10243	5	11	NULL	NULL	NULL	HBO1	GP		is a type of					MYST protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_64_2_435_s_255	10839822	A fourth human MYST protein is HBO1 (histone acetyltransferase bound  to ORC), which was discovered in a two-hybrid screen on the basis of its interaction with the ORC1 subunit of the origin recognition complex (ORC) ( ).	bind
43610	3	10243	5	11	NULL	NULL	NULL	HBO1	GP	human	interact with					ORC	GP		ORC1 subunit		NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_64_2_435_s_255	10839822	A fourth human MYST protein is HBO1 (histone acetyltransferase bound  to ORC), which was discovered in a two-hybrid screen on the basis of its interaction with the ORC1 subunit of the origin recognition complex (ORC) ( ).	bind
43611	4	10243	5	11	NULL	NULL	NULL	ORC	GP		is					origin recognition complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_64_2_435_s_255	10839822	A fourth human MYST protein is HBO1 (histone acetyltransferase bound  to ORC), which was discovered in a two-hybrid screen on the basis of its interaction with the ORC1 subunit of the origin recognition complex (ORC) ( ).	bind
36484	1	10243	6	10	NULL	0	NULL	HBO1	NULL		is a type of	NULL				MYST protein	NULL				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_64_2_435_s_255	10839822	A fourth human MYST protein is HBO1 (histone acetyltransferase bound  to ORC), which was discovered in a two-hybrid screen on the basis of its interaction with the ORC1 subunit of the origin recognition complex (ORC) ( ).	bind
36485	2	10243	6	10	NULL	0	NULL	HBO1	NULL	human	bind	NULL				ORC	NULL		ORC1 subunit		NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_64_2_435_s_255	10839822	A fourth human MYST protein is HBO1 (histone acetyltransferase bound  to ORC), which was discovered in a two-hybrid screen on the basis of its interaction with the ORC1 subunit of the origin recognition complex (ORC) ( ).	bind
36486	3	10243	6	NULL	NULL	0	NULL	ORC	NULL		is	NULL				origin recognition complex	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_64_2_435_s_255	10839822	A fourth human MYST protein is HBO1 (histone acetyltransferase bound  to ORC), which was discovered in a two-hybrid screen on the basis of its interaction with the ORC1 subunit of the origin recognition complex (ORC) ( ).	bind
48427	4	10243	6	10	NULL	0	NULL	HBO1	NULL		is	NULL				histone acetyltransferase bound to ORC	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_64_2_435_s_255	10839822	A fourth human MYST protein is HBO1 (histone acetyltransferase bound  to ORC), which was discovered in a two-hybrid screen on the basis of its interaction with the ORC1 subunit of the origin recognition complex (ORC) ( ).	bind
43612	1	10245	5	11	NULL	NULL	NULL	growth factors	GP		bind					cell-membrane receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_31_18456_s_225	8702490	A fourth hypothesis invokes differences in the binding of growth factors to their cell-membrane receptors, which in several instances requires the presence of heparan sulfate, leading to a change in cell proliferation ( 36).	bind
43613	2	10245	5	11	NULL	NULL	NULL	statement 1	Process		requires					heparan sulfate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_31_18456_s_225	8702490	A fourth hypothesis invokes differences in the binding of growth factors to their cell-membrane receptors, which in several instances requires the presence of heparan sulfate, leading to a change in cell proliferation ( 36).	bind
43614	3	10245	5	11	NULL	NULL	NULL	statement 2	Process		leads to					cell proliferation	Process	change in			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_31_18456_s_225	8702490	A fourth hypothesis invokes differences in the binding of growth factors to their cell-membrane receptors, which in several instances requires the presence of heparan sulfate, leading to a change in cell proliferation ( 36).	bind
36487	1	10245	6	NULL	NULL	0	NULL	growth factors	NULL		bind	NULL				cell membrane receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_31_18456_s_225	8702490	A fourth hypothesis invokes differences in the binding of growth factors to their cell-membrane receptors, which in several instances requires the presence of heparan sulfate, leading to a change in cell proliferation ( 36).	bind
36488	2	10245	6	NULL	NULL	0	NULL	statement 1	NULL		requires	NULL				heparan sulfate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_31_18456_s_225	8702490	A fourth hypothesis invokes differences in the binding of growth factors to their cell-membrane receptors, which in several instances requires the presence of heparan sulfate, leading to a change in cell proliferation ( 36).	bind
36489	3	10245	6	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				cell proliferation	NULL	change in			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_31_18456_s_225	8702490	A fourth hypothesis invokes differences in the binding of growth factors to their cell-membrane receptors, which in several instances requires the presence of heparan sulfate, leading to a change in cell proliferation ( 36).	bind
43615	1	10246	5	11	NULL	NULL	NULL	TM1	GP		is					transmembrane one	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_50_32016_s_58	8943250	A fourth mutation that converted a leucine to a serine in transmembrane one (TM1 L-S) destroyed the binding of iodinated Orphanin FQ.	bind
48728	2	10246	5	11	NULL	NULL	NULL	TM1	GP		is converted to			leucine		TM1	GP		serine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_50_32016_s_58	8943250	A fourth mutation that converted a leucine to a serine in transmembrane one (TM1 L-S) destroyed the binding of iodinated Orphanin FQ.	bind
48729	3	10246	5	11	NULL	NULL	NULL	TM1	GP		bind					Orphanin FQ	GP	iodinated			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_50_32016_s_58	8943250	A fourth mutation that converted a leucine to a serine in transmembrane one (TM1 L-S) destroyed the binding of iodinated Orphanin FQ.	bind
48730	4	10246	5	11	NULL	NULL	NULL	statement 2	Process		destroys					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_50_32016_s_58	8943250	A fourth mutation that converted a leucine to a serine in transmembrane one (TM1 L-S) destroyed the binding of iodinated Orphanin FQ.	bind
36490	1	10246	6	NULL	NULL	0	NULL	TM1	NULL		is	NULL				transmembrane one	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_50_32016_s_58	8943250	A fourth mutation that converted a leucine to a serine in transmembrane one (TM1 L-S) destroyed the binding of iodinated Orphanin FQ.	bind
36491	2	10246	6	NULL	NULL	0	NULL	TM-1	NULL		is converted to	NULL		leucine		TM-1	NULL		serine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_50_32016_s_58	8943250	A fourth mutation that converted a leucine to a serine in transmembrane one (TM1 L-S) destroyed the binding of iodinated Orphanin FQ.	bind
36492	3	10246	6	NULL	NULL	0	NULL	TM1	NULL		bind	NULL				Orphanin FQ	NULL	iodinated			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_50_32016_s_58	8943250	A fourth mutation that converted a leucine to a serine in transmembrane one (TM1 L-S) destroyed the binding of iodinated Orphanin FQ.	bind
36493	4	10246	6	NULL	NULL	0	NULL	statement 2	NULL		destroys	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_50_32016_s_58	8943250	A fourth mutation that converted a leucine to a serine in transmembrane one (TM1 L-S) destroyed the binding of iodinated Orphanin FQ.	bind
43616	1	10247	5	11	NULL	NULL	NULL	anti- Candida antibodies	GP		bind					Candida	Organism				NULL	lavage fluid	NULL	NULL	NULL	NULL	gw60_infectimmun_70_10_5790_s_200	12228309	A fourth possibility is that, due to infection with  Candida, anti- Candida antibodies could be bound by  Candida in the lavage fluid and removed during processing for the soluble fraction.	bind
36494	1	10247	6	NULL	NULL	0	NULL	anti- Candida antibodies	NULL		bind	NULL				Candida	NULL				NULL	lavage fluid	0	NULL	NULL	NULL	gw60_infectimmun_70_10_5790_s_200	12228309	A fourth possibility is that, due to infection with  Candida, anti- Candida antibodies could be bound by  Candida in the lavage fluid and removed during processing for the soluble fraction.	bind
43623	1	10249	5	11	NULL	NULL	NULL	Jak3 probe	GP		bind					CD3zeta	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_25378_s_170	11349123	A fraction (~1/150) of Jak3 probe bound to CD3zeta ( lane 4).	bind
36496	1	10249	6	NULL	NULL	0	NULL	Jak3 probe	NULL		bind	NULL				CD3zeta	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_27_25378_s_170	11349123	A fraction (~1/150) of Jak3 probe bound to CD3zeta ( lane 4).	bind
43624	1	10250	5	11	NULL	NULL	NULL	CDK7	GP		bind					XPD	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_14_3749_s_36	11447116	A fraction of CDK7 is also bound to XPD (Figure  1A), which is found along with CAK in TFIIH.	bind
43627	2	10250	5	11	NULL	NULL	NULL	XPD	GP		is found in					TFIIH	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_14_3749_s_36	11447116	A fraction of CDK7 is also bound to XPD (Figure  1A), which is found along with CAK in TFIIH.	bind
43628	3	10250	5	11	NULL	NULL	NULL	CAK	GP		is found in					TFIIH	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_14_3749_s_36	11447116	A fraction of CDK7 is also bound to XPD (Figure  1A), which is found along with CAK in TFIIH.	bind
36497	1	10250	6	NULL	NULL	0	NULL	CDK7	NULL		bind	NULL				XPD	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_20_14_3749_s_36	11447116	A fraction of CDK7 is also bound to XPD (Figure  1A), which is found along with CAK in TFIIH.	bind
37016	2	10250	6	NULL	NULL	0	NULL	XPD	NULL		is found in	NULL				TFIIH	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_20_14_3749_s_36	11447116	A fraction of CDK7 is also bound to XPD (Figure  1A), which is found along with CAK in TFIIH.	bind
37017	3	10250	6	NULL	NULL	0	NULL	CAK	NULL		is found in	NULL				TFIIH	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_20_14_3749_s_36	11447116	A fraction of CDK7 is also bound to XPD (Figure  1A), which is found along with CAK in TFIIH.	bind
43630	1	10251	5	11	NULL	NULL	NULL	LS-Rg	GP		bind					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_science_261_5120_7687382_s_6	7687382	A fraction of commercial  heparin bound to LS-Rg and LS-Rg bound to heparin-agarose, both in a calcium-dependent  manner.	bind
43631	2	10251	5	11	NULL	NULL	NULL	statement 1	Process		is dependent on					calcium	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_science_261_5120_7687382_s_6	7687382	A fraction of commercial  heparin bound to LS-Rg and LS-Rg bound to heparin-agarose, both in a calcium-dependent  manner.	bind
36498	1	10251	6	NULL	NULL	0	NULL	heparin	NULL		bind	NULL				LS-Rg	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_science_261_5120_7687382_s_6	7687382	A fraction of commercial  heparin bound to LS-Rg and LS-Rg bound to heparin-agarose, both in a calcium-dependent  manner.	bind
36499	2	10251	6	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				calcium	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_science_261_5120_7687382_s_6	7687382	A fraction of commercial  heparin bound to LS-Rg and LS-Rg bound to heparin-agarose, both in a calcium-dependent  manner.	bind
43634	1	10252	5	11	NULL	NULL	NULL	CREB polypeptide	GP		bind					GST-KIX	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_2_3_353_s_105	9774973	A fraction of each CREB polypeptide bound to GST-KIX resin is shown.	bind
36500	1	10252	6	NULL	NULL	0	NULL	CREB polypeptide	NULL		bind	NULL				GST-KIX	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_2_3_353_s_105	9774973	A fraction of each CREB polypeptide bound to GST-KIX resin is shown.	bind
43635	1	10253	5	11	NULL	NULL	NULL	mtHsp70	GP		bind		transiently			Tim44	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_5_941_s_14	11230118	A fraction of mtHsp70 transiently binds to the inner membrane protein Tim44 in an ATP-sensitive manner ( Kronidou  et al., 1994;  Rassow  et al., 1994;  Schneider  et al., 1994;  von Ahsen  et al., 1995;  Ungermann  et al., 1996).	bind
43636	2	10253	5	11	NULL	NULL	NULL	Tim44	GP		is a type of					inner membrane protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_5_941_s_14	11230118	A fraction of mtHsp70 transiently binds to the inner membrane protein Tim44 in an ATP-sensitive manner ( Kronidou  et al., 1994;  Rassow  et al., 1994;  Schneider  et al., 1994;  von Ahsen  et al., 1995;  Ungermann  et al., 1996).	bind
43637	3	10253	5	11	NULL	NULL	NULL	statement 1	Process		is sensitive to					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_5_941_s_14	11230118	A fraction of mtHsp70 transiently binds to the inner membrane protein Tim44 in an ATP-sensitive manner ( Kronidou  et al., 1994;  Rassow  et al., 1994;  Schneider  et al., 1994;  von Ahsen  et al., 1995;  Ungermann  et al., 1996).	bind
36501	1	10253	6	NULL	NULL	0	NULL	Tim44	NULL		is a type of	NULL				inner membrane protein	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_20_5_941_s_14	11230118	A fraction of mtHsp70 transiently binds to the inner membrane protein Tim44 in an ATP-sensitive manner ( Kronidou  et al., 1994;  Rassow  et al., 1994;  Schneider  et al., 1994;  von Ahsen  et al., 1995;  Ungermann  et al., 1996).	bind
36502	2	10253	6	NULL	NULL	0	NULL	mtHsp70	NULL		bind	NULL	transiently			Tim44	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_20_5_941_s_14	11230118	A fraction of mtHsp70 transiently binds to the inner membrane protein Tim44 in an ATP-sensitive manner ( Kronidou  et al., 1994;  Rassow  et al., 1994;  Schneider  et al., 1994;  von Ahsen  et al., 1995;  Ungermann  et al., 1996).	bind
36503	3	10253	6	NULL	NULL	0	NULL	statement 1	NULL		is sensitive to	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_20_5_941_s_14	11230118	A fraction of mtHsp70 transiently binds to the inner membrane protein Tim44 in an ATP-sensitive manner ( Kronidou  et al., 1994;  Rassow  et al., 1994;  Schneider  et al., 1994;  von Ahsen  et al., 1995;  Ungermann  et al., 1996).	bind
43639	1	10254	5	11	NULL	NULL	NULL	Smc3 fragment	GP		does not bind			251-968		chitin matrix	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_6_765_s_238	12654244	A fraction of Smc3's central aa 251-968 fragment was not bound to the chitin matrix, presumably because a portion of the Smc1/Smc3 heterodimer is not bound to Scc1 (see   Figure 3C).	bind
43641	2	10254	5	11	NULL	NULL	NULL	Smc1/Smc3 heterodimer	GP		does not bind					Scc1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_6_765_s_238	12654244	A fraction of Smc3's central aa 251-968 fragment was not bound to the chitin matrix, presumably because a portion of the Smc1/Smc3 heterodimer is not bound to Scc1 (see   Figure 3C).	bind
43642	3	10254	5	11	NULL	NULL	NULL	statement 2	Process		leads to		possibly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_6_765_s_238	12654244	A fraction of Smc3's central aa 251-968 fragment was not bound to the chitin matrix, presumably because a portion of the Smc1/Smc3 heterodimer is not bound to Scc1 (see   Figure 3C).	bind
36504	1	10254	6	NULL	NULL	0	NULL	Smc1/Smc3 heterodimer	NULL		does not bind	NULL				Scc1	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_112_6_765_s_238	12654244	A fraction of Smc3's central aa 251-968 fragment was not bound to the chitin matrix, presumably because a portion of the Smc1/Smc3 heterodimer is not bound to Scc1 (see   Figure 3C).	bind
36505	2	10254	6	10	NULL	0	NULL	Smc3 fragment			does not bind			251-968		chitin					NULL		NULL	NULL	NULL	NULL	gw60_cell_112_6_765_s_238	12654244	A fraction of Smc3's central aa 251-968 fragment was not bound to the chitin matrix, presumably because a portion of the Smc1/Smc3 heterodimer is not bound to Scc1 (see   Figure 3C).	bind
48428	3	10254	6	10	NULL	0	NULL	statement 1	NULL		leads to	NULL	possibly			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_112_6_765_s_238	12654244	A fraction of Smc3's central aa 251-968 fragment was not bound to the chitin matrix, presumably because a portion of the Smc1/Smc3 heterodimer is not bound to Scc1 (see   Figure 3C).	bind
43644	1	10255	5	11	NULL	NULL	NULL	U2 snRNA	NucleicAcid		bind					Cus1p	GP				NULL	splicing extracts	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2176_s_157	10688664	A fraction of U2 snRNA is bound to Cus1p in splicing extracts.	bind
36506	1	10255	6	NULL	NULL	0	NULL	U2 snRNA	NULL		bind	NULL				Cus1p	NULL				NULL	splicing extracts	0	NULL	NULL	NULL	gw60_molcellbiol_20_6_2176_s_157	10688664	A fraction of U2 snRNA is bound to Cus1p in splicing extracts.	bind
43646	1	10256	5	11	NULL	NULL	NULL	U3 fragment	GP		bind			3' domain		U3-55k	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_18_3462_s_193	10982864	A fragment consisting of the entire 3' domain of U3 was bound by U3-55k  in vivo (Fig.  4, 3' Domain, lanes 1 - 3), but as expected U3-55k did not interact with a sub-fragment consisting of the Box C''/D motif (composed of U3 Box C'', Box D and flanking stems; Fig.  4, lanes 7 - 9).	bind
43648	2	10256	5	11	NULL	NULL	NULL	U3-55k	GP		does not interact with					sub-fragment	AminoAcid		Box C''/D motif		NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_18_3462_s_193	10982864	A fragment consisting of the entire 3' domain of U3 was bound by U3-55k  in vivo (Fig.  4, 3' Domain, lanes 1 - 3), but as expected U3-55k did not interact with a sub-fragment consisting of the Box C''/D motif (composed of U3 Box C'', Box D and flanking stems; Fig.  4, lanes 7 - 9).	bind
43650	3	10256	5	11	NULL	NULL	NULL	sub-fragment	AminoAcid		is composed of			Box C''/D motif					U3 Box C''		NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_18_3462_s_193	10982864	A fragment consisting of the entire 3' domain of U3 was bound by U3-55k  in vivo (Fig.  4, 3' Domain, lanes 1 - 3), but as expected U3-55k did not interact with a sub-fragment consisting of the Box C''/D motif (composed of U3 Box C'', Box D and flanking stems; Fig.  4, lanes 7 - 9).	bind
43653	4	10256	5	11	NULL	NULL	NULL	sub-fragment	AminoAcid		is composed of			Box C''/D motif					Box D		NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_18_3462_s_193	10982864	A fragment consisting of the entire 3' domain of U3 was bound by U3-55k  in vivo (Fig.  4, 3' Domain, lanes 1 - 3), but as expected U3-55k did not interact with a sub-fragment consisting of the Box C''/D motif (composed of U3 Box C'', Box D and flanking stems; Fig.  4, lanes 7 - 9).	bind
43654	5	10256	5	11	NULL	NULL	NULL	sub-fragment	AminoAcid		is composed of			Box C''/D motif					flanking stems		NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_18_3462_s_193	10982864	A fragment consisting of the entire 3' domain of U3 was bound by U3-55k  in vivo (Fig.  4, 3' Domain, lanes 1 - 3), but as expected U3-55k did not interact with a sub-fragment consisting of the Box C''/D motif (composed of U3 Box C'', Box D and flanking stems; Fig.  4, lanes 7 - 9).	bind
36507	1	10256	6	NULL	NULL	0	NULL	U3	NULL		bind	NULL		3' domain		U3-55k	NULL				NULL	in vivo	0	NULL	NULL	NULL	gw60_nucleicacidsres_28_18_3462_s_193	10982864	A fragment consisting of the entire 3' domain of U3 was bound by U3-55k  in vivo (Fig.  4, 3' Domain, lanes 1 - 3), but as expected U3-55k did not interact with a sub-fragment consisting of the Box C''/D motif (composed of U3 Box C'', Box D and flanking stems; Fig.  4, lanes 7 - 9).	bind
36508	2	10256	6	10	NULL	0	NULL	U3-55k			does not interact with					sub-fragment			Box C''/D motif		NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_18_3462_s_193	10982864	A fragment consisting of the entire 3' domain of U3 was bound by U3-55k  in vivo (Fig.  4, 3' Domain, lanes 1 - 3), but as expected U3-55k did not interact with a sub-fragment consisting of the Box C''/D motif (composed of U3 Box C'', Box D and flanking stems; Fig.  4, lanes 7 - 9).	bind
48430	3	10256	6	10	NULL	0	NULL	sub-fragment			is composed of			Box C''/D motif					U3 Box C''		NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_18_3462_s_193	10982864	A fragment consisting of the entire 3' domain of U3 was bound by U3-55k  in vivo (Fig.  4, 3' Domain, lanes 1 - 3), but as expected U3-55k did not interact with a sub-fragment consisting of the Box C''/D motif (composed of U3 Box C'', Box D and flanking stems; Fig.  4, lanes 7 - 9).	bind
48431	4	10256	6	10	NULL	0	NULL	sub-fragment			is composed of			Box C''/D motif					Box D		NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_18_3462_s_193	10982864	A fragment consisting of the entire 3' domain of U3 was bound by U3-55k  in vivo (Fig.  4, 3' Domain, lanes 1 - 3), but as expected U3-55k did not interact with a sub-fragment consisting of the Box C''/D motif (composed of U3 Box C'', Box D and flanking stems; Fig.  4, lanes 7 - 9).	bind
48432	5	10256	6	10	NULL	0	NULL	sub-fragment			is composed of			Box C''/D motif					flanking stem		NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_18_3462_s_193	10982864	A fragment consisting of the entire 3' domain of U3 was bound by U3-55k  in vivo (Fig.  4, 3' Domain, lanes 1 - 3), but as expected U3-55k did not interact with a sub-fragment consisting of the Box C''/D motif (composed of U3 Box C'', Box D and flanking stems; Fig.  4, lanes 7 - 9).	bind
44241	1	10257	5	11	NULL	NULL	NULL	fragment	GP		contains					ATP-DnaA	GP			box b	NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_6169_s_113	10545126	A fragment containing ATP-DnaA box b and ATP-DnaA box c, but without DnaA boxes 1 and 2, did not show any binding of ATP- and ADP-DnaA protein.	bind
44242	2	10257	5	11	NULL	NULL	NULL	fragment	GP		contains					ATP-DnaA	GP			box c	NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_6169_s_113	10545126	A fragment containing ATP-DnaA box b and ATP-DnaA box c, but without DnaA boxes 1 and 2, did not show any binding of ATP- and ADP-DnaA protein.	bind
44243	3	10257	5	11	NULL	NULL	NULL	fragment	GP		does not contain					DnaA	GP			box 1	NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_6169_s_113	10545126	A fragment containing ATP-DnaA box b and ATP-DnaA box c, but without DnaA boxes 1 and 2, did not show any binding of ATP- and ADP-DnaA protein.	bind
44244	4	10257	5	11	NULL	NULL	NULL	fragment	GP		does not contain					DnaA	GP			box 2	NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_6169_s_113	10545126	A fragment containing ATP-DnaA box b and ATP-DnaA box c, but without DnaA boxes 1 and 2, did not show any binding of ATP- and ADP-DnaA protein.	bind
44245	5	10257	5	11	NULL	NULL	NULL	statement 1	GP		does not bind					ATP-DnaA protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_6169_s_113	10545126	A fragment containing ATP-DnaA box b and ATP-DnaA box c, but without DnaA boxes 1 and 2, did not show any binding of ATP- and ADP-DnaA protein.	bind
44246	6	10257	5	11	NULL	NULL	NULL	statement 2	GP		does not bind					ATP-DnaA protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_6169_s_113	10545126	A fragment containing ATP-DnaA box b and ATP-DnaA box c, but without DnaA boxes 1 and 2, did not show any binding of ATP- and ADP-DnaA protein.	bind
44247	7	10257	5	11	NULL	NULL	NULL	statement 3	GP		does not bind					ATP-DnaA protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_6169_s_113	10545126	A fragment containing ATP-DnaA box b and ATP-DnaA box c, but without DnaA boxes 1 and 2, did not show any binding of ATP- and ADP-DnaA protein.	bind
44248	8	10257	5	11	NULL	NULL	NULL	statement 4	GP		does not bind					ATP-DnaA protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_6169_s_113	10545126	A fragment containing ATP-DnaA box b and ATP-DnaA box c, but without DnaA boxes 1 and 2, did not show any binding of ATP- and ADP-DnaA protein.	bind
44249	9	10257	5	11	NULL	NULL	NULL	statement 1	GP		does not bind					ADP-DnaA protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_6169_s_113	10545126	A fragment containing ATP-DnaA box b and ATP-DnaA box c, but without DnaA boxes 1 and 2, did not show any binding of ATP- and ADP-DnaA protein.	bind
44250	10	10257	5	11	NULL	NULL	NULL	statement 2	GP		does not bind					ADP-DnaA protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_6169_s_113	10545126	A fragment containing ATP-DnaA box b and ATP-DnaA box c, but without DnaA boxes 1 and 2, did not show any binding of ATP- and ADP-DnaA protein.	bind
44251	11	10257	5	11	NULL	NULL	NULL	statement 3	GP		does not bind					ADP-DnaA protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_6169_s_113	10545126	A fragment containing ATP-DnaA box b and ATP-DnaA box c, but without DnaA boxes 1 and 2, did not show any binding of ATP- and ADP-DnaA protein.	bind
44252	12	10257	5	11	NULL	NULL	NULL	statement 4	GP		does not bind					ADP-DnaA protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_6169_s_113	10545126	A fragment containing ATP-DnaA box b and ATP-DnaA box c, but without DnaA boxes 1 and 2, did not show any binding of ATP- and ADP-DnaA protein.	bind
37018	1	10257	6	NULL	NULL	0	NULL	fragment containing ATP-DnaA box b	NULL		does not bind	NULL				ATP-DnaA protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_6169_s_113	10545126	A fragment containing ATP-DnaA box b and ATP-DnaA box c, but without DnaA boxes 1 and 2, did not show any binding of ATP- and ADP-DnaA protein.	bind
37019	2	10257	6	NULL	NULL	0	NULL	fragment containing ATP-DnaA box c	NULL		does not bind	NULL				ATP-DnaA protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_6169_s_113	10545126	A fragment containing ATP-DnaA box b and ATP-DnaA box c, but without DnaA boxes 1 and 2, did not show any binding of ATP- and ADP-DnaA protein.	bind
48550	3	10257	6	NULL	NULL	0	NULL	statement 1	NULL		occurs simultaneously with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_18_21_6169_s_113	10545126	A fragment containing ATP-DnaA box b and ATP-DnaA box c, but without DnaA boxes 1 and 2, did not show any binding of ATP- and ADP-DnaA protein.	bind
48551	4	10257	6	NULL	NULL	0	NULL	fragment containing ATP-DnaA box b	NULL		does not bind	NULL				ATP-DnaA protein	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_18_21_6169_s_113	10545126	A fragment containing ATP-DnaA box b and ATP-DnaA box c, but without DnaA boxes 1 and 2, did not show any binding of ATP- and ADP-DnaA protein.	bind
48552	5	10257	6	NULL	NULL	0	NULL	fragment containing ATP-DnaA box c	NULL		does not bind	NULL				ADP-DnaA protein	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_18_21_6169_s_113	10545126	A fragment containing ATP-DnaA box b and ATP-DnaA box c, but without DnaA boxes 1 and 2, did not show any binding of ATP- and ADP-DnaA protein.	bind
48553	6	10257	6	NULL	NULL	0	NULL	statement 4	NULL		occurs simultaneously with	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_18_21_6169_s_113	10545126	A fragment containing ATP-DnaA box b and ATP-DnaA box c, but without DnaA boxes 1 and 2, did not show any binding of ATP- and ADP-DnaA protein.	bind
48554	7	10257	6	NULL	NULL	0	NULL	fragment without DnaA box1	NULL		does not bind	NULL				ATP-DnaA protein	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_18_21_6169_s_113	10545126	A fragment containing ATP-DnaA box b and ATP-DnaA box c, but without DnaA boxes 1 and 2, did not show any binding of ATP- and ADP-DnaA protein.	bind
48555	8	10257	6	NULL	NULL	0	NULL	fragment without DnaA box 2	NULL		does not bind	NULL				ATP-DnaA protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_6169_s_113	10545126	A fragment containing ATP-DnaA box b and ATP-DnaA box c, but without DnaA boxes 1 and 2, did not show any binding of ATP- and ADP-DnaA protein.	bind
48556	9	10257	6	NULL	NULL	0	NULL	statement 7	NULL		occurs simultaneously with	NULL				statement 8	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_18_21_6169_s_113	10545126	A fragment containing ATP-DnaA box b and ATP-DnaA box c, but without DnaA boxes 1 and 2, did not show any binding of ATP- and ADP-DnaA protein.	bind
48557	10	10257	6	NULL	NULL	0	NULL	fragment containing ATP-DnaA box b	NULL		does not bind	NULL				ADP-DnaA protein	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_18_21_6169_s_113	10545126	A fragment containing ATP-DnaA box b and ATP-DnaA box c, but without DnaA boxes 1 and 2, did not show any binding of ATP- and ADP-DnaA protein.	bind
48558	11	10257	6	NULL	NULL	0	NULL	fragment containing ATP-DnaA box c	NULL		does not bind	NULL				ADP-DnaA protein	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_18_21_6169_s_113	10545126	A fragment containing ATP-DnaA box b and ATP-DnaA box c, but without DnaA boxes 1 and 2, did not show any binding of ATP- and ADP-DnaA protein.	bind
48559	12	10257	6	NULL	NULL	0	NULL	statement 10	NULL		occurs simultaneously with	NULL				statement 11	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_18_21_6169_s_113	10545126	A fragment containing ATP-DnaA box b and ATP-DnaA box c, but without DnaA boxes 1 and 2, did not show any binding of ATP- and ADP-DnaA protein.	bind
43657	1	10258	5	11	NULL	NULL	NULL	fragment containing part of coil X	GP		does not bind					p115	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_14_10196_s_84	10744704	A fragment containing part of coil X ( lane 3), a fragment containing coil II ( lane 5), and GST alone ( lane 1) did not bind p115.	bind
43659	2	10258	5	11	NULL	NULL	NULL	fragment containing coil II 	GP		does not bind					p115	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_14_10196_s_84	10744704	A fragment containing part of coil X ( lane 3), a fragment containing coil II ( lane 5), and GST alone ( lane 1) did not bind p115.	bind
43660	3	10258	5	11	NULL	NULL	NULL	GST	GP		does not bind					p115	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_14_10196_s_84	10744704	A fragment containing part of coil X ( lane 3), a fragment containing coil II ( lane 5), and GST alone ( lane 1) did not bind p115.	bind
36509	1	10258	6	NULL	NULL	0	NULL	fragment containing part of coil X	NULL		does not bind	NULL				p115	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_14_10196_s_84	10744704	A fragment containing part of coil X ( lane 3), a fragment containing coil II ( lane 5), and GST alone ( lane 1) did not bind p115.	bind
36510	2	10258	6	NULL	NULL	0	NULL	fragment containing coil II	NULL		does not bind	NULL				p115	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_14_10196_s_84	10744704	A fragment containing part of coil X ( lane 3), a fragment containing coil II ( lane 5), and GST alone ( lane 1) did not bind p115.	bind
36511	3	10258	6	NULL	NULL	0	NULL	GST	NULL		does not bind	NULL				p115	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_14_10196_s_84	10744704	A fragment containing part of coil X ( lane 3), a fragment containing coil II ( lane 5), and GST alone ( lane 1) did not bind p115.	bind
43661	1	10259	5	11	NULL	NULL	NULL	AP53	Organism		is					PAM-expressing group A streptococcal strain	Organism				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_38_24420_s_66	9733732	A fragment encompassing K1-K3 bound to the PAM-expressing group A streptococcal strain AP53, whereas fragments containing K4 alone or K5 and the proteinase domain (m-Pg) showed almost no binding to this strain (Fig.  2,  A-C).	bind
43662	2	10259	5	11	NULL	NULL	NULL	fragment	AminoAcid		encompass								K1-K3		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_38_24420_s_66	9733732	A fragment encompassing K1-K3 bound to the PAM-expressing group A streptococcal strain AP53, whereas fragments containing K4 alone or K5 and the proteinase domain (m-Pg) showed almost no binding to this strain (Fig.  2,  A-C).	bind
43663	3	10259	5	11	NULL	NULL	NULL	statement 2	AminoAcid		bind					AP53	Organism				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_38_24420_s_66	9733732	A fragment encompassing K1-K3 bound to the PAM-expressing group A streptococcal strain AP53, whereas fragments containing K4 alone or K5 and the proteinase domain (m-Pg) showed almost no binding to this strain (Fig.  2,  A-C).	bind
43664	4	10259	5	11	NULL	NULL	NULL	fragment	AminoAcid		contains								K4		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_38_24420_s_66	9733732	A fragment encompassing K1-K3 bound to the PAM-expressing group A streptococcal strain AP53, whereas fragments containing K4 alone or K5 and the proteinase domain (m-Pg) showed almost no binding to this strain (Fig.  2,  A-C).	bind
43665	5	10259	5	11	NULL	NULL	NULL	statement 4	AminoAcid		does not bind					AP53	Organism				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_38_24420_s_66	9733732	A fragment encompassing K1-K3 bound to the PAM-expressing group A streptococcal strain AP53, whereas fragments containing K4 alone or K5 and the proteinase domain (m-Pg) showed almost no binding to this strain (Fig.  2,  A-C).	bind
43667	6	10259	5	11	NULL	NULL	NULL	fragment	AminoAcid		contains								K5		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_38_24420_s_66	9733732	A fragment encompassing K1-K3 bound to the PAM-expressing group A streptococcal strain AP53, whereas fragments containing K4 alone or K5 and the proteinase domain (m-Pg) showed almost no binding to this strain (Fig.  2,  A-C).	bind
43669	7	10259	5	11	NULL	NULL	NULL	statement 6	AminoAcid		does not bind					AP53	Organism				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_38_24420_s_66	9733732	A fragment encompassing K1-K3 bound to the PAM-expressing group A streptococcal strain AP53, whereas fragments containing K4 alone or K5 and the proteinase domain (m-Pg) showed almost no binding to this strain (Fig.  2,  A-C).	bind
43670	8	10259	5	11	NULL	NULL	NULL	fragment	AminoAcid		contains								m-Pg		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_38_24420_s_66	9733732	A fragment encompassing K1-K3 bound to the PAM-expressing group A streptococcal strain AP53, whereas fragments containing K4 alone or K5 and the proteinase domain (m-Pg) showed almost no binding to this strain (Fig.  2,  A-C).	bind
43672	9	10259	5	11	NULL	NULL	NULL	m-Pg	GP		is					proteinase domain	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_38_24420_s_66	9733732	A fragment encompassing K1-K3 bound to the PAM-expressing group A streptococcal strain AP53, whereas fragments containing K4 alone or K5 and the proteinase domain (m-Pg) showed almost no binding to this strain (Fig.  2,  A-C).	bind
43673	10	10259	5	11	NULL	NULL	NULL	statement 8	AminoAcid		does not bind					AP53	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_38_24420_s_66	9733732	A fragment encompassing K1-K3 bound to the PAM-expressing group A streptococcal strain AP53, whereas fragments containing K4 alone or K5 and the proteinase domain (m-Pg) showed almost no binding to this strain (Fig.  2,  A-C).	bind
36512	1	10259	6	NULL	NULL	0	NULL		NULL		bind	NULL		K1-K3		AP53	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_38_24420_s_66	9733732	A fragment encompassing K1-K3 bound to the PAM-expressing group A streptococcal strain AP53, whereas fragments containing K4 alone or K5 and the proteinase domain (m-Pg) showed almost no binding to this strain (Fig.  2,  A-C).	bind
36513	2	10259	6	NULL	NULL	0	NULL	AP53	NULL		is	NULL				PAM-expressing group A streptococcal strain	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_38_24420_s_66	9733732	A fragment encompassing K1-K3 bound to the PAM-expressing group A streptococcal strain AP53, whereas fragments containing K4 alone or K5 and the proteinase domain (m-Pg) showed almost no binding to this strain (Fig.  2,  A-C).	bind
36514	3	10259	6	NULL	NULL	0	NULL		NULL		does not bind	NULL		K4		AP53	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_38_24420_s_66	9733732	A fragment encompassing K1-K3 bound to the PAM-expressing group A streptococcal strain AP53, whereas fragments containing K4 alone or K5 and the proteinase domain (m-Pg) showed almost no binding to this strain (Fig.  2,  A-C).	bind
36515	4	10259	6	NULL	NULL	0	NULL		NULL		does not bind	NULL		K5		AP53	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_38_24420_s_66	9733732	A fragment encompassing K1-K3 bound to the PAM-expressing group A streptococcal strain AP53, whereas fragments containing K4 alone or K5 and the proteinase domain (m-Pg) showed almost no binding to this strain (Fig.  2,  A-C).	bind
36516	5	10259	6	NULL	NULL	0	NULL		NULL		does not bind	NULL		proteinase domain		AP53	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_38_24420_s_66	9733732	A fragment encompassing K1-K3 bound to the PAM-expressing group A streptococcal strain AP53, whereas fragments containing K4 alone or K5 and the proteinase domain (m-Pg) showed almost no binding to this strain (Fig.  2,  A-C).	bind
43674	2	10260	5	11	NULL	NULL	NULL	p3RIZrdeltaNBam construct	GP		bind			1272-1706		PR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_26_15933_s_153	9632640	A fragment encompassing residues 900 to 1272 (construct p3RIZrBB) did not bind to GST-PR, but a fragment encoding residues 1272 to the end codon 1706 (construct p3RIZrdeltaNBam) retained full PR binding activity.	bind
43677	1	10260	5	11	NULL	NULL	NULL	p3RIZrBB construct	GP		does not bind			900-1272		GST-PR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_26_15933_s_153	9632640	A fragment encompassing residues 900 to 1272 (construct p3RIZrBB) did not bind to GST-PR, but a fragment encoding residues 1272 to the end codon 1706 (construct p3RIZrdeltaNBam) retained full PR binding activity.	bind
37022	1	10260	6	NULL	NULL	0	NULL	construct p3RIZrBB	NULL		does not bind	NULL		900-1272		GST-PR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_26_15933_s_153	9632640	A fragment encompassing residues 900 to 1272 (construct p3RIZrBB) did not bind to GST-PR, but a fragment encoding residues 1272 to the end codon 1706 (construct p3RIZrdeltaNBam) retained full PR binding activity.	bind
37023	2	10260	6	NULL	NULL	0	NULL	construct p3RIZrdeltaNBam	NULL		bind	NULL		1272-1706		PR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_26_15933_s_153	9632640	A fragment encompassing residues 900 to 1272 (construct p3RIZrBB) did not bind to GST-PR, but a fragment encoding residues 1272 to the end codon 1706 (construct p3RIZrdeltaNBam) retained full PR binding activity.	bind
43683	1	10262	5	11	NULL	NULL	NULL	Smad1	GP	mutant	bind			C86-465		calmodulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_52_41430_s_178	11007779	A fragment lacking the amino-terminal 86 residues (Smad1(C86-465)) still bound calmodulin, while deleting nine more amino acids (Smad1(C95-465)) eliminated calmodulin binding (Fig.  2,  A and  B).	bind
43684	2	10262	5	11	NULL	NULL	NULL	Smad1	GP	mutant	does not bind			C95-465		calmodulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_52_41430_s_178	11007779	A fragment lacking the amino-terminal 86 residues (Smad1(C86-465)) still bound calmodulin, while deleting nine more amino acids (Smad1(C95-465)) eliminated calmodulin binding (Fig.  2,  A and  B).	bind
36517	1	10262	6	10	NULL	0	NULL	Smad1	NULL	mutant	bind	NULL		C86-485		calmodulin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_52_41430_s_178	11007779	A fragment lacking the amino-terminal 86 residues (Smad1(C86-465)) still bound calmodulin, while deleting nine more amino acids (Smad1(C95-465)) eliminated calmodulin binding (Fig.  2,  A and  B).	bind
36518	2	10262	6	10	NULL	0	NULL	Smad1	NULL	mutant	does not bind	NULL		C95-465		calmodulin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_52_41430_s_178	11007779	A fragment lacking the amino-terminal 86 residues (Smad1(C86-465)) still bound calmodulin, while deleting nine more amino acids (Smad1(C95-465)) eliminated calmodulin binding (Fig.  2,  A and  B).	bind
43685	1	10263	5	11	NULL	NULL	NULL	APC fragment	GP		contains								beta-catenin-binding repeat 7;;SAMP repeat		NULL		NULL	NULL	NULL	NULL	gw60_embo_19_10_2270_s_57	10811618	A fragment of APC containing beta-catenin-binding repeat 7 and the third SAMP repeat bound equally well to the Axin-RGS and p38 proteins (Figure  2A).	bind
43686	2	10263	5	11	NULL	NULL	NULL	statement 1	GP		bind					Axin-RGS	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_10_2270_s_57	10811618	A fragment of APC containing beta-catenin-binding repeat 7 and the third SAMP repeat bound equally well to the Axin-RGS and p38 proteins (Figure  2A).	bind
43687	3	10263	5	11	NULL	NULL	NULL	statement 1	GP		bind					p38 proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_10_2270_s_57	10811618	A fragment of APC containing beta-catenin-binding repeat 7 and the third SAMP repeat bound equally well to the Axin-RGS and p38 proteins (Figure  2A).	bind
36519	2	10263	6	10	NULL	0	NULL	statement 1			bind					Axin-RGS					NULL		NULL	NULL	NULL	NULL	gw60_embo_19_10_2270_s_57	10811618	A fragment of APC containing beta-catenin-binding repeat 7 and the third SAMP repeat bound equally well to the Axin-RGS and p38 proteins (Figure  2A).	bind
36520	3	10263	6	10	NULL	0	NULL	statement 1			bind					p38 proteins					NULL		NULL	NULL	NULL	NULL	gw60_embo_19_10_2270_s_57	10811618	A fragment of APC containing beta-catenin-binding repeat 7 and the third SAMP repeat bound equally well to the Axin-RGS and p38 proteins (Figure  2A).	bind
57486	1	10263	6	10	NULL	0	NULL	APC fragment			contains								\tbeta-catenin-binding repeat 7;;SAMP repeat		NULL		0	NULL	NULL	NULL	gw60_embo_19_10_2270_s_57	10811618	A fragment of APC containing beta-catenin-binding repeat 7 and the third SAMP repeat bound equally well to the Axin-RGS and p38 proteins (Figure  2A).	bind
43688	1	10264	5	11	NULL	NULL	NULL	CKIIbeta fragment	GP		does not bind					Mos	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_17_9136_s_94	9256448	A fragment of CKIIbeta that does not bind to Mos, CKIIbeta1-160, had no effect ( 7).	bind
36521	1	10264	6	10	NULL	0	NULL	CKIIbeta fragment			does not bind					Mos					NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_17_9136_s_94	9256448	A fragment of CKIIbeta that does not bind to Mos, CKIIbeta1-160, had no effect ( 7).	bind
44235	1	10265	5	11	NULL	NULL	NULL	hCASK fragment	GP		contains							intact	SH3 domain;;GUK domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_52_41192_s_221	10993877	A fragment of hCASK containing the intact SH3 and GUK domains ( SH3GUK) does not bind the hCASK SH3 domain, again suggesting that SH3-GUK interactions in  cis are inhibitory to similar interactions in  trans.	bind
44239	3	10265	5	11	NULL	NULL	NULL	statement 1	GP		does not bind					hCASK	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_52_41192_s_221	10993877	A fragment of hCASK containing the intact SH3 and GUK domains ( SH3GUK) does not bind the hCASK SH3 domain, again suggesting that SH3-GUK interactions in  cis are inhibitory to similar interactions in  trans.	bind
57487	2	10265	5	11	NULL	NULL	NULL	SH3GUK	GP		is					intact SH3 and GUK domains	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_52_41192_s_221	10993877	A fragment of hCASK containing the intact SH3 and GUK domains ( SH3GUK) does not bind the hCASK SH3 domain, again suggesting that SH3-GUK interactions in  cis are inhibitory to similar interactions in  trans.	bind
37024	1	10265	6	NULL	NULL	0	NULL	hCASK	NULL		does not bind	NULL		SH3GUK		hCASK	NULL		SH3 domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_52_41192_s_221	10993877	A fragment of hCASK containing the intact SH3 and GUK domains ( SH3GUK) does not bind the hCASK SH3 domain, again suggesting that SH3-GUK interactions in  cis are inhibitory to similar interactions in  trans.	bind
37025	2	10265	6	NULL	NULL	0	NULL	SH3GUK	NULL		is 	NULL				intact SH3 and GUK domains	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_52_41192_s_221	10993877	A fragment of hCASK containing the intact SH3 and GUK domains ( SH3GUK) does not bind the hCASK SH3 domain, again suggesting that SH3-GUK interactions in  cis are inhibitory to similar interactions in  trans.	bind
43690	1	10266	5	11	NULL	NULL	NULL	hEST1A fragment	GP		contains			630-1388					TPR repeats;;PIN domain		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_13_8_698_s_80	12699629	A fragment of hEST1A (spanning aa 630-1388) that contained the TPR repeats and PIN domain did not bind DNA (Figure S2A).	bind
43691	2	10266	5	11	NULL	NULL	NULL	statement 1	GP		does not bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_13_8_698_s_80	12699629	A fragment of hEST1A (spanning aa 630-1388) that contained the TPR repeats and PIN domain did not bind DNA (Figure S2A).	bind
36522	1	10266	6	10	NULL	0	NULL	hEST1A	NULL		contains	NULL		aa 630-1388			NULL		TPR repeats;; PIN domain		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_13_8_698_s_80	12699629	A fragment of hEST1A (spanning aa 630-1388) that contained the TPR repeats and PIN domain did not bind DNA (Figure S2A).	bind
36523	2	10266	6	10	NULL	0	NULL	statement 1	NULL		does not bind	NULL				DNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_13_8_698_s_80	12699629	A fragment of hEST1A (spanning aa 630-1388) that contained the TPR repeats and PIN domain did not bind DNA (Figure S2A).	bind
43692	1	10267	5	11	NULL	NULL	NULL	MASP-1 fragment	GP		comprise								CUB-1;;EGF		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_28_25894_s_173	11337510	A fragment of MASP-1 comprising the CUB-1 and EGF modules ( 13) bound to MBP-A, demonstrating that either or both of these domains form part of the binding site.	bind
43693	2	10267	5	11	NULL	NULL	NULL	statement 1	GP		bind					MBP-A	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_28_25894_s_173	11337510	A fragment of MASP-1 comprising the CUB-1 and EGF modules ( 13) bound to MBP-A, demonstrating that either or both of these domains form part of the binding site.	bind
36524	1	10267	6	NULL	NULL	0	NULL	MASP-1	NULL		bind	NULL		CUB-1;; EGF		MBP-A	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_28_25894_s_173	11337510	A fragment of MASP-1 comprising the CUB-1 and EGF modules ( 13) bound to MBP-A, demonstrating that either or both of these domains form part of the binding site.	bind
44226	1	10268	5	11	NULL	NULL	NULL	N-WASP fragment	GP		include								basic region		NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_70_0_649_s_269	11395419	A fragment of N-WASP including this basic region and GBD binds PIP2-containing vesicles, and deletion or point mutations reducing the positive charge of the basic region reduce PIP2 binding ( 66,  86).	bind
44227	2	10268	5	11	NULL	NULL	NULL	N-WASP fragment	GP		include								GBD		NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_70_0_649_s_269	11395419	A fragment of N-WASP including this basic region and GBD binds PIP2-containing vesicles, and deletion or point mutations reducing the positive charge of the basic region reduce PIP2 binding ( 66,  86).	bind
44228	3	10268	5	11	NULL	NULL	NULL	vesicles	CellComponent		contains					PIP2	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_70_0_649_s_269	11395419	A fragment of N-WASP including this basic region and GBD binds PIP2-containing vesicles, and deletion or point mutations reducing the positive charge of the basic region reduce PIP2 binding ( 66,  86).	bind
44229	4	10268	5	11	NULL	NULL	NULL	statement 1	GP		bind					statement 3	GP				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_70_0_649_s_269	11395419	A fragment of N-WASP including this basic region and GBD binds PIP2-containing vesicles, and deletion or point mutations reducing the positive charge of the basic region reduce PIP2 binding ( 66,  86).	bind
44230	5	10268	5	11	NULL	NULL	NULL	statement 2	GP		bind					statement 3	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_70_0_649_s_269	11395419	A fragment of N-WASP including this basic region and GBD binds PIP2-containing vesicles, and deletion or point mutations reducing the positive charge of the basic region reduce PIP2 binding ( 66,  86).	bind
44231	6	10268	5	11	NULL	NULL	NULL	N-WASP	GP	deletion mutation of	reduce							positive charge of	basic region		NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_70_0_649_s_269	11395419	A fragment of N-WASP including this basic region and GBD binds PIP2-containing vesicles, and deletion or point mutations reducing the positive charge of the basic region reduce PIP2 binding ( 66,  86).	bind
44232	7	10268	5	11	NULL	NULL	NULL	N-WASP fragment	GP	point mutation of	reduce							positive charge of	basic region		NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_70_0_649_s_269	11395419	A fragment of N-WASP including this basic region and GBD binds PIP2-containing vesicles, and deletion or point mutations reducing the positive charge of the basic region reduce PIP2 binding ( 66,  86).	bind
44233	8	10268	5	11	NULL	NULL	NULL	statement 6	Process		reduce					PIP2	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_70_0_649_s_269	11395419	A fragment of N-WASP including this basic region and GBD binds PIP2-containing vesicles, and deletion or point mutations reducing the positive charge of the basic region reduce PIP2 binding ( 66,  86).	bind
44234	9	10268	5	11	NULL	NULL	NULL	statement 7	Process		reduce					PIP2	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_70_0_649_s_269	11395419	A fragment of N-WASP including this basic region and GBD binds PIP2-containing vesicles, and deletion or point mutations reducing the positive charge of the basic region reduce PIP2 binding ( 66,  86).	bind
37026	1	10268	6	NULL	NULL	0	NULL	N-WASP	NULL		bind	NULL		basic region		PIP2-containing vesicles	NULL				NULL		0	NULL	NULL	NULL	gw60_annrevbiochem_70_0_649_s_269	11395419	A fragment of N-WASP including this basic region and GBD binds PIP2-containing vesicles, and deletion or point mutations reducing the positive charge of the basic region reduce PIP2 binding ( 66,  86).	bind
37027	2	10268	6	NULL	NULL	0	NULL	N-WASP	NULL		bind	NULL		GBD		PIP2-containing vesicles	NULL				NULL		0	NULL	NULL	NULL	gw60_annrevbiochem_70_0_649_s_269	11395419	A fragment of N-WASP including this basic region and GBD binds PIP2-containing vesicles, and deletion or point mutations reducing the positive charge of the basic region reduce PIP2 binding ( 66,  86).	bind
37028	3	10268	6	NULL	NULL	0	NULL	statement 1	NULL		is simultaneous with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_annrevbiochem_70_0_649_s_269	11395419	A fragment of N-WASP including this basic region and GBD binds PIP2-containing vesicles, and deletion or point mutations reducing the positive charge of the basic region reduce PIP2 binding ( 66,  86).	bind
37029	4	10268	6	NULL	NULL	0	NULL	N-WASP	NULL	deletion of	reduces	NULL		basic region		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_annrevbiochem_70_0_649_s_269	11395419	A fragment of N-WASP including this basic region and GBD binds PIP2-containing vesicles, and deletion or point mutations reducing the positive charge of the basic region reduce PIP2 binding ( 66,  86).	bind
48569	5	10268	6	NULL	NULL	0	NULL	N-WASP	NULL	mutant	reduces	NULL					NULL	positive charge on	basic region		NULL		0	NULL	NULL	NULL	gw60_annrevbiochem_70_0_649_s_269	11395419	A fragment of N-WASP including this basic region and GBD binds PIP2-containing vesicles, and deletion or point mutations reducing the positive charge of the basic region reduce PIP2 binding ( 66,  86).	bind
48570	6	10268	6	NULL	NULL	0	NULL	statement 5	NULL		reduces	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_annrevbiochem_70_0_649_s_269	11395419	A fragment of N-WASP including this basic region and GBD binds PIP2-containing vesicles, and deletion or point mutations reducing the positive charge of the basic region reduce PIP2 binding ( 66,  86).	bind
43694	1	10270	5	11	NULL	NULL	NULL	PEX5 fragment	GP		contains							little more than	PTS1-binding domain		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_147_4_761_s_184	10562279	A fragment of PEX5 containing little more than the PTS1-binding domain of PEX5 retained full binding to PEX12.	bind
43696	2	10270	5	11	NULL	NULL	NULL	statement 1	GP		bind					PEX12	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_147_4_761_s_184	10562279	A fragment of PEX5 containing little more than the PTS1-binding domain of PEX5 retained full binding to PEX12.	bind
36525	1	10270	6	10	NULL	0	NULL	PEX5 fragment			contains								PTS1-binding domain		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_147_4_761_s_184	10562279	A fragment of PEX5 containing little more than the PTS1-binding domain of PEX5 retained full binding to PEX12.	bind
57488	2	10270	6	10	NULL	0	NULL	statement 1			bind					PEX12					NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_4_761_s_184	10562279	A fragment of PEX5 containing little more than the PTS1-binding domain of PEX5 retained full binding to PEX12.	bind
43697	1	10271	5	11	NULL	NULL	NULL	Raf kinase fragment	GP		bind		preferentially			GTP-Ras	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_29_22037_s_224	10801823	A fragment of Raf kinase that binds preferentially to GTP-Ras was used as an affinity reagent to isolate active Ha-Ras proteins from stimulated cells.	bind
36526	1	10271	6	NULL	NULL	0	NULL	fragment of Raf kinase	NULL		bind	NULL	preferentially			GTP-Ras	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_29_22037_s_224	10801823	A fragment of Raf kinase that binds preferentially to GTP-Ras was used as an affinity reagent to isolate active Ha-Ras proteins from stimulated cells.	bind
44217	1	10272	5	11	NULL	NULL	NULL	T antigen fragment	GP		express								J domain		NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_2_179_s_505	12040123	A fragment of T antigen that expresses the J domain and pRB-binding motif (N1 to 121) is sufficient to induce pancreatic and hepatic tumors as well as full-length T antigen, suggesting that binding to p53 is not required to induce tumors in these systems ( 7,  241).	bind
44218	2	10272	5	11	NULL	NULL	NULL	T antigen fragment	GP		express								pRB-binding motif (N1 to 121)		NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_2_179_s_505	12040123	A fragment of T antigen that expresses the J domain and pRB-binding motif (N1 to 121) is sufficient to induce pancreatic and hepatic tumors as well as full-length T antigen, suggesting that binding to p53 is not required to induce tumors in these systems ( 7,  241).	bind
44219	3	10272	5	11	NULL	NULL	NULL	statement 1	Process		induce					pancreatic tumor	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_2_179_s_505	12040123	A fragment of T antigen that expresses the J domain and pRB-binding motif (N1 to 121) is sufficient to induce pancreatic and hepatic tumors as well as full-length T antigen, suggesting that binding to p53 is not required to induce tumors in these systems ( 7,  241).	bind
44220	4	10272	5	11	NULL	NULL	NULL	statement 2	Process		induce					pancreatic tumor	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_2_179_s_505	12040123	A fragment of T antigen that expresses the J domain and pRB-binding motif (N1 to 121) is sufficient to induce pancreatic and hepatic tumors as well as full-length T antigen, suggesting that binding to p53 is not required to induce tumors in these systems ( 7,  241).	bind
44221	5	10272	5	11	NULL	NULL	NULL	statement 1	Process		induce					hepatic tumor	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_2_179_s_505	12040123	A fragment of T antigen that expresses the J domain and pRB-binding motif (N1 to 121) is sufficient to induce pancreatic and hepatic tumors as well as full-length T antigen, suggesting that binding to p53 is not required to induce tumors in these systems ( 7,  241).	bind
44222	6	10272	5	11	NULL	NULL	NULL	statement 2	Process		induce					hepatic tumor	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_2_179_s_505	12040123	A fragment of T antigen that expresses the J domain and pRB-binding motif (N1 to 121) is sufficient to induce pancreatic and hepatic tumors as well as full-length T antigen, suggesting that binding to p53 is not required to induce tumors in these systems ( 7,  241).	bind
48560	1	10272	6	NULL	NULL	0	NULL	fragment of T antigen	NULL		expresses	NULL					NULL		J domain		NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_2_179_s_505	12040123	A fragment of T antigen that expresses the J domain and pRB-binding motif (N1 to 121) is sufficient to induce pancreatic and hepatic tumors as well as full-length T antigen, suggesting that binding to p53 is not required to induce tumors in these systems ( 7,  241).	bind
48561	2	10272	6	NULL	NULL	0	NULL	fragment of T antigen	NULL		expresses	NULL					NULL		pRB-binding motif (N1-121)		NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_2_179_s_505	12040123	A fragment of T antigen that expresses the J domain and pRB-binding motif (N1 to 121) is sufficient to induce pancreatic and hepatic tumors as well as full-length T antigen, suggesting that binding to p53 is not required to induce tumors in these systems ( 7,  241).	bind
48562	3	10272	6	NULL	NULL	0	NULL	statement 1	NULL		induce	NULL				pancreatic tumors	NULL				NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_2_179_s_505	12040123	A fragment of T antigen that expresses the J domain and pRB-binding motif (N1 to 121) is sufficient to induce pancreatic and hepatic tumors as well as full-length T antigen, suggesting that binding to p53 is not required to induce tumors in these systems ( 7,  241).	bind
48563	4	10272	6	NULL	NULL	0	NULL	statement 2	NULL		induce	NULL				pancreatic tumors	NULL				NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_2_179_s_505	12040123	A fragment of T antigen that expresses the J domain and pRB-binding motif (N1 to 121) is sufficient to induce pancreatic and hepatic tumors as well as full-length T antigen, suggesting that binding to p53 is not required to induce tumors in these systems ( 7,  241).	bind
48564	5	10272	6	NULL	NULL	0	NULL	statement 1	NULL		induce	NULL				hepatic tumors	NULL				NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_2_179_s_505	12040123	A fragment of T antigen that expresses the J domain and pRB-binding motif (N1 to 121) is sufficient to induce pancreatic and hepatic tumors as well as full-length T antigen, suggesting that binding to p53 is not required to induce tumors in these systems ( 7,  241).	bind
48565	6	10272	6	NULL	NULL	0	NULL	statement 2	NULL		induce	NULL				hepatic tumors	NULL				NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_2_179_s_505	12040123	A fragment of T antigen that expresses the J domain and pRB-binding motif (N1 to 121) is sufficient to induce pancreatic and hepatic tumors as well as full-length T antigen, suggesting that binding to p53 is not required to induce tumors in these systems ( 7,  241).	bind
44196	1	10273	5	11	NULL	NULL	NULL	Nt-TPR9	GP		is					N terminus to the end of TPR9	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_142	16880507	A fragment of Tfc4 extending from the N terminus to the end of TPR9 (Nt-TPR9) binds to Brf1 with reduced affinity relative to the two independent Brf1 binding sites (Nt-TPR5 and TPR6-9) contained within this region ( ).	bind
44212	2	10273	5	11	NULL	NULL	NULL	Tfc4 fragment	GP		bind			Nt-TPR9		Brf1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_142	16880507	A fragment of Tfc4 extending from the N terminus to the end of TPR9 (Nt-TPR9) binds to Brf1 with reduced affinity relative to the two independent Brf1 binding sites (Nt-TPR5 and TPR6-9) contained within this region ( ).	bind
44213	3	10273	5	11	NULL	NULL	NULL	Tfc4	GP		bind			Nt-TPR5		Brf1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_142	16880507	A fragment of Tfc4 extending from the N terminus to the end of TPR9 (Nt-TPR9) binds to Brf1 with reduced affinity relative to the two independent Brf1 binding sites (Nt-TPR5 and TPR6-9) contained within this region ( ).	bind
44214	4	10273	5	11	NULL	NULL	NULL	Tfc4	GP		bind			TPR6-9		Brf1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_142	16880507	A fragment of Tfc4 extending from the N terminus to the end of TPR9 (Nt-TPR9) binds to Brf1 with reduced affinity relative to the two independent Brf1 binding sites (Nt-TPR5 and TPR6-9) contained within this region ( ).	bind
44215	5	10273	5	11	NULL	NULL	NULL	statement 2	Process	affinity of	is lower than					statement 3	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_142	16880507	A fragment of Tfc4 extending from the N terminus to the end of TPR9 (Nt-TPR9) binds to Brf1 with reduced affinity relative to the two independent Brf1 binding sites (Nt-TPR5 and TPR6-9) contained within this region ( ).	bind
44216	6	10273	5	11	NULL	NULL	NULL	statement 2	Process	affinity of	is lower than					statement 4	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_142	16880507	A fragment of Tfc4 extending from the N terminus to the end of TPR9 (Nt-TPR9) binds to Brf1 with reduced affinity relative to the two independent Brf1 binding sites (Nt-TPR5 and TPR6-9) contained within this region ( ).	bind
37030	1	10273	6	NULL	NULL	0	NULL	Nt-TPR9	NULL		is	NULL				N terminus to the end of TPR9	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_142	16880507	A fragment of Tfc4 extending from the N terminus to the end of TPR9 (Nt-TPR9) binds to Brf1 with reduced affinity relative to the two independent Brf1 binding sites (Nt-TPR5 and TPR6-9) contained within this region ( ).	bind
37031	2	10273	6	NULL	NULL	0	NULL	Tfc4	NULL		bind	NULL		Nt-TPR9		Brf1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_142	16880507	A fragment of Tfc4 extending from the N terminus to the end of TPR9 (Nt-TPR9) binds to Brf1 with reduced affinity relative to the two independent Brf1 binding sites (Nt-TPR5 and TPR6-9) contained within this region ( ).	bind
37032	3	10273	6	NULL	NULL	0	NULL	Tfc4	NULL		bind	NULL		Nt-TPR5		Brf1	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_142	16880507	A fragment of Tfc4 extending from the N terminus to the end of TPR9 (Nt-TPR9) binds to Brf1 with reduced affinity relative to the two independent Brf1 binding sites (Nt-TPR5 and TPR6-9) contained within this region ( ).	bind
37033	4	10273	6	NULL	NULL	0	NULL	Tfc4	NULL		bind	NULL		TPR6-9		Brf1	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_142	16880507	A fragment of Tfc4 extending from the N terminus to the end of TPR9 (Nt-TPR9) binds to Brf1 with reduced affinity relative to the two independent Brf1 binding sites (Nt-TPR5 and TPR6-9) contained within this region ( ).	bind
37034	5	10273	6	NULL	NULL	0	NULL	statement 2	NULL	affinity of	is lower than	NULL				statement 3	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_142	16880507	A fragment of Tfc4 extending from the N terminus to the end of TPR9 (Nt-TPR9) binds to Brf1 with reduced affinity relative to the two independent Brf1 binding sites (Nt-TPR5 and TPR6-9) contained within this region ( ).	bind
37035	6	10273	6	NULL	NULL	0	NULL	statement 2	NULL	affinity of	is lower than	NULL				statement 4	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_142	16880507	A fragment of Tfc4 extending from the N terminus to the end of TPR9 (Nt-TPR9) binds to Brf1 with reduced affinity relative to the two independent Brf1 binding sites (Nt-TPR5 and TPR6-9) contained within this region ( ).	bind
43705	1	10274	5	11	NULL	NULL	NULL	Rb protein fragment	GP		bind					MCM7	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_9_1007_s_52	15879550	A fragment of the Rb protein that binds MCM7 and inhibits helicase activity (Sterner et al. 1998 ) blocks unwinding, as do neutralizing antibodies to CDC45, which functions as a cofactor for the MCM complex (Pacek and Walter 2004 ).	bind
43706	2	10274	5	11	NULL	NULL	NULL	statement 1	Process		inhibit					helicase	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_9_1007_s_52	15879550	A fragment of the Rb protein that binds MCM7 and inhibits helicase activity (Sterner et al. 1998 ) blocks unwinding, as do neutralizing antibodies to CDC45, which functions as a cofactor for the MCM complex (Pacek and Walter 2004 ).	bind
43708	3	10274	5	11	NULL	NULL	NULL	statement 2	Process		block					unwinding	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_9_1007_s_52	15879550	A fragment of the Rb protein that binds MCM7 and inhibits helicase activity (Sterner et al. 1998 ) blocks unwinding, as do neutralizing antibodies to CDC45, which functions as a cofactor for the MCM complex (Pacek and Walter 2004 ).	bind
43710	4	10274	5	11	NULL	NULL	NULL	CDC45	GP		acts as a 					cofactor	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_9_1007_s_52	15879550	A fragment of the Rb protein that binds MCM7 and inhibits helicase activity (Sterner et al. 1998 ) blocks unwinding, as do neutralizing antibodies to CDC45, which functions as a cofactor for the MCM complex (Pacek and Walter 2004 ).	bind
48433	5	10274	5	11	NULL	NULL	NULL	statement 4	Process		occurs in					MCM complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_9_1007_s_52	15879550	A fragment of the Rb protein that binds MCM7 and inhibits helicase activity (Sterner et al. 1998 ) blocks unwinding, as do neutralizing antibodies to CDC45, which functions as a cofactor for the MCM complex (Pacek and Walter 2004 ).	bind
36578	1	10274	6	NULL	NULL	0	NULL	fragment of Rb protein	NULL		bind	NULL				MCM7	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_9_1007_s_52	15879550	A fragment of the Rb protein that binds MCM7 and inhibits helicase activity (Sterner et al. 1998 ) blocks unwinding, as do neutralizing antibodies to CDC45, which functions as a cofactor for the MCM complex (Pacek and Walter 2004 ).	bind
36579	2	10274	6	NULL	NULL	0	NULL	statement 1	NULL		inhibits	NULL				helicase	NULL	activity of			NULL		0	NULL	NULL	NULL	gw70_genesdev_19_9_1007_s_52	15879550	A fragment of the Rb protein that binds MCM7 and inhibits helicase activity (Sterner et al. 1998 ) blocks unwinding, as do neutralizing antibodies to CDC45, which functions as a cofactor for the MCM complex (Pacek and Walter 2004 ).	bind
36580	3	10274	6	NULL	NULL	0	NULL	statement 1	NULL		blocks	NULL				DNA unwinding activity	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_9_1007_s_52	15879550	A fragment of the Rb protein that binds MCM7 and inhibits helicase activity (Sterner et al. 1998 ) blocks unwinding, as do neutralizing antibodies to CDC45, which functions as a cofactor for the MCM complex (Pacek and Walter 2004 ).	bind
36581	4	10274	6	10	NULL	0	NULL	CDC45	NULL		acts as a 	NULL				cofactor	NULL				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_9_1007_s_52	15879550	A fragment of the Rb protein that binds MCM7 and inhibits helicase activity (Sterner et al. 1998 ) blocks unwinding, as do neutralizing antibodies to CDC45, which functions as a cofactor for the MCM complex (Pacek and Walter 2004 ).	bind
48434	5	10274	6	10	NULL	0	NULL	statement 4	NULL		occurs in	NULL				MCM complex	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_9_1007_s_52	15879550	A fragment of the Rb protein that binds MCM7 and inhibits helicase activity (Sterner et al. 1998 ) blocks unwinding, as do neutralizing antibodies to CDC45, which functions as a cofactor for the MCM complex (Pacek and Walter 2004 ).	bind
43701	1	10275	5	11	NULL	NULL	NULL				contains			reductase domain fragment				only	FMN domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_10_8827_s_255	14681230	A fragment of the reductase domain containing only the FMN domain could bind caveolin-1, suggesting that the FMN domain itself is essential for the caveolin-1 interaction.	bind
43702	2	10275	5	11	NULL	NULL	NULL	statement 1	GP		bind					caveolin-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_10_8827_s_255	14681230	A fragment of the reductase domain containing only the FMN domain could bind caveolin-1, suggesting that the FMN domain itself is essential for the caveolin-1 interaction.	bind
43703	3	10275	5	11	NULL	NULL	NULL				is essential for			FMN domain		caveolin-1	GP	interaction of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_10_8827_s_255	14681230	A fragment of the reductase domain containing only the FMN domain could bind caveolin-1, suggesting that the FMN domain itself is essential for the caveolin-1 interaction.	bind
36582	1	10275	6	10	NULL	0	NULL	reductase domain fragment	NULL		contains	NULL					NULL		FMN domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_10_8827_s_255	14681230	A fragment of the reductase domain containing only the FMN domain could bind caveolin-1, suggesting that the FMN domain itself is essential for the caveolin-1 interaction.	bind
36583	3	10275	6	10	NULL	0	NULL		NULL		is essential for	NULL		FMN domain		caveolin-1	NULL	interaction of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_10_8827_s_255	14681230	A fragment of the reductase domain containing only the FMN domain could bind caveolin-1, suggesting that the FMN domain itself is essential for the caveolin-1 interaction.	bind
48435	2	10275	6	10	NULL	0	NULL	statement 1	NULL		bind	NULL				caveolin-1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_10_8827_s_255	14681230	A fragment of the reductase domain containing only the FMN domain could bind caveolin-1, suggesting that the FMN domain itself is essential for the caveolin-1 interaction.	bind
43725	1	10276	5	11	NULL	NULL	NULL	free peptide	AminoAcid	amino acid sequence of	is identical to					phage	Organism				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_11_7075_s_41	16423833	A free peptide with identical amino acid sequence to that displayed by the phage was able to inhibit binding of the phage to SC, suggesting that the peptide alone was sufficient for binding.	bind
43726	2	10276	5	11	NULL	NULL	NULL	phage	Organism		bind					SC	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_11_7075_s_41	16423833	A free peptide with identical amino acid sequence to that displayed by the phage was able to inhibit binding of the phage to SC, suggesting that the peptide alone was sufficient for binding.	bind
43727	3	10276	5	11	NULL	NULL	NULL	statement 1	Process		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_11_7075_s_41	16423833	A free peptide with identical amino acid sequence to that displayed by the phage was able to inhibit binding of the phage to SC, suggesting that the peptide alone was sufficient for binding.	bind
36584	1	10276	6	NULL	NULL	0	NULL	phage	NULL		bind	NULL				SC	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_11_7075_s_41	16423833	A free peptide with identical amino acid sequence to that displayed by the phage was able to inhibit binding of the phage to SC, suggesting that the peptide alone was sufficient for binding.	bind
36585	2	10276	6	10	NULL	0	NULL	free peptide	NULL	amino acid sequence of 	is identical to	NULL				phage	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_11_7075_s_41	16423833	A free peptide with identical amino acid sequence to that displayed by the phage was able to inhibit binding of the phage to SC, suggesting that the peptide alone was sufficient for binding.	bind
36586	3	10276	6	NULL	NULL	0	NULL	statement 2	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_11_7075_s_41	16423833	A free peptide with identical amino acid sequence to that displayed by the phage was able to inhibit binding of the phage to SC, suggesting that the peptide alone was sufficient for binding.	bind
43730	1	10277	5	11	NULL	NULL	NULL	oligosaccharide	Chemical	core 	is attached to		freshly			glycoprotein	GP	unfolded			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_14_13607_s_22	14732712	A freshly attached core oligosaccharide of an unfolded glycoprotein is first trimmed by glucosidases I and II, after which the glycoprotein becomes bound to CNX or CRT, this being followed by binding of the complex to ERp57 ( ,  ).	bind
43731	2	10277	5	11	NULL	NULL	NULL	statement 1	GP		is trimmed by					glucosidases I	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_14_13607_s_22	14732712	A freshly attached core oligosaccharide of an unfolded glycoprotein is first trimmed by glucosidases I and II, after which the glycoprotein becomes bound to CNX or CRT, this being followed by binding of the complex to ERp57 ( ,  ).	bind
43732	3	10277	5	11	NULL	NULL	NULL	statement 1	GP		is trimmed by					glucosidases II	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_14_13607_s_22	14732712	A freshly attached core oligosaccharide of an unfolded glycoprotein is first trimmed by glucosidases I and II, after which the glycoprotein becomes bound to CNX or CRT, this being followed by binding of the complex to ERp57 ( ,  ).	bind
43733	4	10277	5	11	NULL	NULL	NULL	glycoprotein	GP		bind					CNX	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_14_13607_s_22	14732712	A freshly attached core oligosaccharide of an unfolded glycoprotein is first trimmed by glucosidases I and II, after which the glycoprotein becomes bound to CNX or CRT, this being followed by binding of the complex to ERp57 ( ,  ).	bind
43734	5	10277	5	11	NULL	NULL	NULL	glycoprotein	GP		bind					CRT	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_14_13607_s_22	14732712	A freshly attached core oligosaccharide of an unfolded glycoprotein is first trimmed by glucosidases I and II, after which the glycoprotein becomes bound to CNX or CRT, this being followed by binding of the complex to ERp57 ( ,  ).	bind
43735	6	10277	5	11	NULL	NULL	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_14_13607_s_22	14732712	A freshly attached core oligosaccharide of an unfolded glycoprotein is first trimmed by glucosidases I and II, after which the glycoprotein becomes bound to CNX or CRT, this being followed by binding of the complex to ERp57 ( ,  ).	bind
43736	7	10277	5	11	NULL	NULL	NULL	statement 2	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_14_13607_s_22	14732712	A freshly attached core oligosaccharide of an unfolded glycoprotein is first trimmed by glucosidases I and II, after which the glycoprotein becomes bound to CNX or CRT, this being followed by binding of the complex to ERp57 ( ,  ).	bind
43737	8	10277	5	11	NULL	NULL	NULL	statement 2	Process		leads to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_14_13607_s_22	14732712	A freshly attached core oligosaccharide of an unfolded glycoprotein is first trimmed by glucosidases I and II, after which the glycoprotein becomes bound to CNX or CRT, this being followed by binding of the complex to ERp57 ( ,  ).	bind
43738	9	10277	5	11	NULL	NULL	NULL	statement 3	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_14_13607_s_22	14732712	A freshly attached core oligosaccharide of an unfolded glycoprotein is first trimmed by glucosidases I and II, after which the glycoprotein becomes bound to CNX or CRT, this being followed by binding of the complex to ERp57 ( ,  ).	bind
43739	10	10277	5	11	NULL	NULL	NULL	statement 3	Process		leads to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_14_13607_s_22	14732712	A freshly attached core oligosaccharide of an unfolded glycoprotein is first trimmed by glucosidases I and II, after which the glycoprotein becomes bound to CNX or CRT, this being followed by binding of the complex to ERp57 ( ,  ).	bind
43740	11	10277	5	11	NULL	NULL	NULL	statement 4	GP		bind					ERp57	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_14_13607_s_22	14732712	A freshly attached core oligosaccharide of an unfolded glycoprotein is first trimmed by glucosidases I and II, after which the glycoprotein becomes bound to CNX or CRT, this being followed by binding of the complex to ERp57 ( ,  ).	bind
43741	12	10277	5	11	NULL	NULL	NULL	statement 5	GP		bind					ERp57	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_14_13607_s_22	14732712	A freshly attached core oligosaccharide of an unfolded glycoprotein is first trimmed by glucosidases I and II, after which the glycoprotein becomes bound to CNX or CRT, this being followed by binding of the complex to ERp57 ( ,  ).	bind
37036	1	10277	6	10	NULL	0	NULL	oligosaccharide		core	is attached to		freshly			glycoprotein		unfolded			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_14_13607_s_22	14732712	A freshly attached core oligosaccharide of an unfolded glycoprotein is first trimmed by glucosidases I and II, after which the glycoprotein becomes bound to CNX or CRT, this being followed by binding of the complex to ERp57 ( ,  ).	bind
37037	2	10277	6	NULL	NULL	0	NULL	glucosidases I	NULL		trims	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_14_13607_s_22	14732712	A freshly attached core oligosaccharide of an unfolded glycoprotein is first trimmed by glucosidases I and II, after which the glycoprotein becomes bound to CNX or CRT, this being followed by binding of the complex to ERp57 ( ,  ).	bind
37038	3	10277	6	NULL	NULL	0	NULL	glucosidase II	NULL		trims	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_14_13607_s_22	14732712	A freshly attached core oligosaccharide of an unfolded glycoprotein is first trimmed by glucosidases I and II, after which the glycoprotein becomes bound to CNX or CRT, this being followed by binding of the complex to ERp57 ( ,  ).	bind
37039	4	10277	6	NULL	NULL	0	NULL	glycoprotein	NULL		bind	NULL				CNX	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_14_13607_s_22	14732712	A freshly attached core oligosaccharide of an unfolded glycoprotein is first trimmed by glucosidases I and II, after which the glycoprotein becomes bound to CNX or CRT, this being followed by binding of the complex to ERp57 ( ,  ).	bind
37040	5	10277	6	NULL	NULL	0	NULL	glycoprotein	NULL		bind	NULL				CRT	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_14_13607_s_22	14732712	A freshly attached core oligosaccharide of an unfolded glycoprotein is first trimmed by glucosidases I and II, after which the glycoprotein becomes bound to CNX or CRT, this being followed by binding of the complex to ERp57 ( ,  ).	bind
37041	6	10277	6	NULL	NULL	0	NULL	statement 4	NULL		is an alternative to	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_14_13607_s_22	14732712	A freshly attached core oligosaccharide of an unfolded glycoprotein is first trimmed by glucosidases I and II, after which the glycoprotein becomes bound to CNX or CRT, this being followed by binding of the complex to ERp57 ( ,  ).	bind
37042	7	10277	6	NULL	NULL	0	NULL	statement 6	NULL		occurs after	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_14_13607_s_22	14732712	A freshly attached core oligosaccharide of an unfolded glycoprotein is first trimmed by glucosidases I and II, after which the glycoprotein becomes bound to CNX or CRT, this being followed by binding of the complex to ERp57 ( ,  ).	bind
37043	8	10277	6	NULL	NULL	0	NULL	statement 6	NULL		occurs after	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_14_13607_s_22	14732712	A freshly attached core oligosaccharide of an unfolded glycoprotein is first trimmed by glucosidases I and II, after which the glycoprotein becomes bound to CNX or CRT, this being followed by binding of the complex to ERp57 ( ,  ).	bind
37044	9	10277	6	NULL	NULL	0	NULL	statement 4	NULL		bind	NULL				ERp57	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_14_13607_s_22	14732712	A freshly attached core oligosaccharide of an unfolded glycoprotein is first trimmed by glucosidases I and II, after which the glycoprotein becomes bound to CNX or CRT, this being followed by binding of the complex to ERp57 ( ,  ).	bind
37045	10	10277	6	NULL	NULL	0	NULL	statement 5	NULL		bind	NULL				ERp57	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_14_13607_s_22	14732712	A freshly attached core oligosaccharide of an unfolded glycoprotein is first trimmed by glucosidases I and II, after which the glycoprotein becomes bound to CNX or CRT, this being followed by binding of the complex to ERp57 ( ,  ).	bind
43742	1	10278	5	11	NULL	NULL	NULL	Rab proteins	GP	mutant	bind		preferentially	S21N		GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_devcell_1_1_73_s_45	11703925	A full-length human RIN1 prey fusion protein  (Han et al., 1997  ) was tested for interaction with bait fusion proteins consisting of wild-type Vps21p and Rab5A, as well as mutant versions of the Rab proteins that preferentially bind GDP (S21N and S34N, respectively).	bind
43743	2	10278	5	11	NULL	NULL	NULL	Rab proteins	GP	mutant	bind		preferentially	S34N		GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_devcell_1_1_73_s_45	11703925	A full-length human RIN1 prey fusion protein  (Han et al., 1997  ) was tested for interaction with bait fusion proteins consisting of wild-type Vps21p and Rab5A, as well as mutant versions of the Rab proteins that preferentially bind GDP (S21N and S34N, respectively).	bind
36587	1	10278	6	NULL	NULL	0	NULL	Rab protein	NULL	mutant	bind	NULL	preferentially	S21N		GDP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_devcell_1_1_73_s_45	11703925	A full-length human RIN1 prey fusion protein  (Han et al., 1997  ) was tested for interaction with bait fusion proteins consisting of wild-type Vps21p and Rab5A, as well as mutant versions of the Rab proteins that preferentially bind GDP (S21N and S34N, respectively).	bind
36588	2	10278	6	NULL	NULL	0	NULL	Rab protein	NULL	mutant	bind	NULL	preferentially	S34N		GDP	NULL				NULL		0	NULL	NULL	NULL	gw60_devcell_1_1_73_s_45	11703925	A full-length human RIN1 prey fusion protein  (Han et al., 1997  ) was tested for interaction with bait fusion proteins consisting of wild-type Vps21p and Rab5A, as well as mutant versions of the Rab proteins that preferentially bind GDP (S21N and S34N, respectively).	bind
43744	1	10279	5	11	NULL	NULL	NULL	MBP	GP		is					maltose binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_5_1225_s_15	11844750	A fuller understanding of how these binding proteins function in transport was realized following our recent observation in the maltose transport system that the periplasmic maltose binding protein (MBP) becomes tightly bound to the membrane transporter (MalFGK2, a complex of MalF, MalG, and two MalK proteins) in the presumed catalytic transition state for ATP hydrolysis ( 22).	bind
43745	2	10279	5	11	NULL	NULL	NULL	MalFGK2	GP		is a type of					membrane transporter	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_5_1225_s_15	11844750	A fuller understanding of how these binding proteins function in transport was realized following our recent observation in the maltose transport system that the periplasmic maltose binding protein (MBP) becomes tightly bound to the membrane transporter (MalFGK2, a complex of MalF, MalG, and two MalK proteins) in the presumed catalytic transition state for ATP hydrolysis ( 22).	bind
43746	3	10279	5	11	NULL	NULL	NULL	MalFGK2	GP		contains					MalF proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_5_1225_s_15	11844750	A fuller understanding of how these binding proteins function in transport was realized following our recent observation in the maltose transport system that the periplasmic maltose binding protein (MBP) becomes tightly bound to the membrane transporter (MalFGK2, a complex of MalF, MalG, and two MalK proteins) in the presumed catalytic transition state for ATP hydrolysis ( 22).	bind
43747	6	10279	5	11	NULL	NULL	NULL	MBP	GP	periplasmic	bind		tightly			MalFGK2	GP				NULL	maltose transport system	NULL	NULL	NULL	NULL	gw60_jbacteriol_184_5_1225_s_15	11844750	A fuller understanding of how these binding proteins function in transport was realized following our recent observation in the maltose transport system that the periplasmic maltose binding protein (MBP) becomes tightly bound to the membrane transporter (MalFGK2, a complex of MalF, MalG, and two MalK proteins) in the presumed catalytic transition state for ATP hydrolysis ( 22).	bind
43812	4	10279	5	11	NULL	NULL	NULL	MalFGK2	GP		contains					MalG proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_5_1225_s_15	11844750	A fuller understanding of how these binding proteins function in transport was realized following our recent observation in the maltose transport system that the periplasmic maltose binding protein (MBP) becomes tightly bound to the membrane transporter (MalFGK2, a complex of MalF, MalG, and two MalK proteins) in the presumed catalytic transition state for ATP hydrolysis ( 22).	bind
43813	5	10279	5	11	NULL	NULL	NULL	MalFGK2	GP		contains					MalK proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_5_1225_s_15	11844750	A fuller understanding of how these binding proteins function in transport was realized following our recent observation in the maltose transport system that the periplasmic maltose binding protein (MBP) becomes tightly bound to the membrane transporter (MalFGK2, a complex of MalF, MalG, and two MalK proteins) in the presumed catalytic transition state for ATP hydrolysis ( 22).	bind
37046	1	10279	6	NULL	NULL	0	NULL	MBP	NULL		is	NULL				maltose binding protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_5_1225_s_15	11844750	A fuller understanding of how these binding proteins function in transport was realized following our recent observation in the maltose transport system that the periplasmic maltose binding protein (MBP) becomes tightly bound to the membrane transporter (MalFGK2, a complex of MalF, MalG, and two MalK proteins) in the presumed catalytic transition state for ATP hydrolysis ( 22).	bind
37047	2	10279	6	10	NULL	0	NULL	MBP		periplasmic	bind		tightly			MalFGK2					NULL	maltose transport system	NULL	NULL	NULL	NULL	gw60_jbacteriol_184_5_1225_s_15	11844750	A fuller understanding of how these binding proteins function in transport was realized following our recent observation in the maltose transport system that the periplasmic maltose binding protein (MBP) becomes tightly bound to the membrane transporter (MalFGK2, a complex of MalF, MalG, and two MalK proteins) in the presumed catalytic transition state for ATP hydrolysis ( 22).	bind
37048	3	10279	6	NULL	NULL	0	NULL	MalFGK2	NULL		is a type of	NULL				membrane transporter	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_5_1225_s_15	11844750	A fuller understanding of how these binding proteins function in transport was realized following our recent observation in the maltose transport system that the periplasmic maltose binding protein (MBP) becomes tightly bound to the membrane transporter (MalFGK2, a complex of MalF, MalG, and two MalK proteins) in the presumed catalytic transition state for ATP hydrolysis ( 22).	bind
37049	4	10279	6	NULL	NULL	0	NULL	statement 2	NULL		occurs in the	NULL				catalytic transition state	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_5_1225_s_15	11844750	A fuller understanding of how these binding proteins function in transport was realized following our recent observation in the maltose transport system that the periplasmic maltose binding protein (MBP) becomes tightly bound to the membrane transporter (MalFGK2, a complex of MalF, MalG, and two MalK proteins) in the presumed catalytic transition state for ATP hydrolysis ( 22).	bind
37050	5	10279	6	NULL	NULL	0	NULL	statement 4	NULL		occurs for	NULL				ATP	NULL	hydrolysis of			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_5_1225_s_15	11844750	A fuller understanding of how these binding proteins function in transport was realized following our recent observation in the maltose transport system that the periplasmic maltose binding protein (MBP) becomes tightly bound to the membrane transporter (MalFGK2, a complex of MalF, MalG, and two MalK proteins) in the presumed catalytic transition state for ATP hydrolysis ( 22).	bind
48571	6	10279	6	NULL	NULL	0	NULL	MalFGK2	NULL		is	NULL				a complex of MalF, MalG, and two MalK proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_5_1225_s_15	11844750	A fuller understanding of how these binding proteins function in transport was realized following our recent observation in the maltose transport system that the periplasmic maltose binding protein (MBP) becomes tightly bound to the membrane transporter (MalFGK2, a complex of MalF, MalG, and two MalK proteins) in the presumed catalytic transition state for ATP hydrolysis ( 22).	bind
43749	1	10280	5	11	NULL	NULL	NULL	TMs	GP		bind		cooperatively			F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_36_22409_s_14	9278391	A function common to all TMs is cooperative binding to F-actin ( 2).	bind
36589	1	10280	6	NULL	NULL	0	NULL	TM	NULL		bind	NULL	cooperatively			F-actin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_36_22409_s_14	9278391	A function common to all TMs is cooperative binding to F-actin ( 2).	bind
43750	1	10281	5	11	NULL	NULL	NULL	DnaJ	GP		bind					DnaK	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_5_2139_s_259	7836443	A Function for the QKRAA Amino Acid Motif: Mediating Binding of DnaJ to DnaK .	bind
48436	2	10281	5	11	NULL	NULL	NULL				mediates			QKRAA Amino Acid Motif		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_5_2139_s_259	7836443	A Function for the QKRAA Amino Acid Motif: Mediating Binding of DnaJ to DnaK .	bind
36590	1	10281	6	NULL	NULL	0	NULL	DnaJ	NULL		bind	NULL				DnaK	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_5_2139_s_259	7836443	A Function for the QKRAA Amino Acid Motif: Mediating Binding of DnaJ to DnaK .	bind
36591	2	10281	6	NULL	NULL	0	NULL		NULL		mediates	NULL		QKRAA amino acid motif		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_5_2139_s_259	7836443	A Function for the QKRAA Amino Acid Motif: Mediating Binding of DnaJ to DnaK .	bind
43753	1	10282	5	11	NULL	NULL	NULL				inhibit			R subunit		kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_12_6687_s_190	9618473	A function for the R subunit apart from kinase inhibition is also suggested by the finding that the cAMP binding domain of RII shares extensive homology with the bacterial catabolite activator protein (CAP) ( 28).	bind
43754	2	10282	5	11	NULL	NULL	NULL	RII	GP		is homologous to		extensively	cAMP binding domain		CAP	GP	bacterial			NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_12_6687_s_190	9618473	A function for the R subunit apart from kinase inhibition is also suggested by the finding that the cAMP binding domain of RII shares extensive homology with the bacterial catabolite activator protein (CAP) ( 28).	bind
43755	3	10282	5	11	NULL	NULL	NULL	CAP	GP		is					catabolite activator protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_12_6687_s_190	9618473	A function for the R subunit apart from kinase inhibition is also suggested by the finding that the cAMP binding domain of RII shares extensive homology with the bacterial catabolite activator protein (CAP) ( 28).	bind
36592	1	10282	6	NULL	NULL	0	NULL	RII	NULL		is homologous to	NULL	extensively	cAMP binding domain		CAP	NULL	bacterial			NULL		0	NULL	NULL	NULL	gw60_pnas_95_12_6687_s_190	9618473	A function for the R subunit apart from kinase inhibition is also suggested by the finding that the cAMP binding domain of RII shares extensive homology with the bacterial catabolite activator protein (CAP) ( 28).	bind
36593	2	10282	6	NULL	NULL	0	NULL	CAP	NULL		is	NULL				catabolite activator protein	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_12_6687_s_190	9618473	A function for the R subunit apart from kinase inhibition is also suggested by the finding that the cAMP binding domain of RII shares extensive homology with the bacterial catabolite activator protein (CAP) ( 28).	bind
36594	3	10282	6	NULL	NULL	0	NULL	R subunit	NULL		functions in	NULL				kinase	NULL	inhibiton of			NULL		0	NULL	NULL	NULL	gw60_pnas_95_12_6687_s_190	9618473	A function for the R subunit apart from kinase inhibition is also suggested by the finding that the cAMP binding domain of RII shares extensive homology with the bacterial catabolite activator protein (CAP) ( 28).	bind
43751	1	10283	5	11	NULL	NULL	NULL	sperm	Cell	free-swimming;;acrosome-reacted;;mouse	does not bind					eggs	Cell	ZP-encased			NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_66_6_1585_s_344	12021035	A function for the ZP3 binding sites on the plasma membrane overlying the acrosome is evident from the fact that free-swimming, acrosome-reacted mouse sperm cannot bind to ZP-encased eggs [ 7.	bind
36595	1	10283	6	10	NULL	0	NULL	sperm	NULL	free swimming;; acrosome-reacted;; mouse	does not bind	NULL				eggs	NULL	ZP-encased			NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_66_6_1585_s_344	12021035	A function for the ZP3 binding sites on the plasma membrane overlying the acrosome is evident from the fact that free-swimming, acrosome-reacted mouse sperm cannot bind to ZP-encased eggs [ 7.	bind
43756	1	10284	5	11	NULL	NULL	NULL	APP	GP	transmembrane	serve as		directly			cell adhesion molecule	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_3_1613_s_216	8576160	A functional  collagen binding site of APP is of great importance, since  transmembrane APP could serve directly as a cell adhesion molecule, and  the secreted forms might be involved in the regulation of cell  interactions.	bind
43758	2	10284	5	11	NULL	NULL	NULL	APP	GP	secreted	is involved in		might be			cell interactions	Process	regulation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_3_1613_s_216	8576160	A functional  collagen binding site of APP is of great importance, since  transmembrane APP could serve directly as a cell adhesion molecule, and  the secreted forms might be involved in the regulation of cell  interactions.	bind
36596	1	10284	6	NULL	NULL	0	NULL	APP	NULL	transmembrane	serves as a	NULL				cell adhesion molecule	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_3_1613_s_216	8576160	A functional  collagen binding site of APP is of great importance, since  transmembrane APP could serve directly as a cell adhesion molecule, and  the secreted forms might be involved in the regulation of cell  interactions.	bind
36597	2	10284	6	NULL	NULL	0	NULL	APP	NULL	secreted form of	is involved in	NULL	might			cell interactions	NULL	regulation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_3_1613_s_216	8576160	A functional  collagen binding site of APP is of great importance, since  transmembrane APP could serve directly as a cell adhesion molecule, and  the secreted forms might be involved in the regulation of cell  interactions.	bind
43759	1	10285	5	11	NULL	NULL	NULL	c-myb gene	GP	functional	is required for					hepatic hematopoiesis	Process	normal;;murine;;fetal			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_24_9203_s_519	11094072	A functional c-myb gene is required for normal murine fetal hepatic hematopoiesis.	bind
36598	1	10285	6	10	NULL	0	NULL	c-myb gene	NULL	functional	is required for	NULL				hepatic hematopoiesis	NULL	normal;; murine;; fetal			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_24_9203_s_519	11094072	A functional c-myb gene is required for normal murine fetal hepatic hematopoiesis.	bind
43761	1	10287	5	11	NULL	NULL	NULL	FnBP fragment	GP	functional	bind					Hsp60	GP	epithelial cell membrane			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_11_6321_s_127	11035741	A functional fragment of FnBP binds to Hsp60 from epithelial cell membrane fractions.	bind
36599	1	10287	6	10	NULL	0	NULL	FnBP fragment	NULL	functional	bind	NULL				Hsp60	NULL	epithelial cell membrane 			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_11_6321_s_127	11035741	A functional fragment of FnBP binds to Hsp60 from epithelial cell membrane fractions.	bind
43762	1	10288	5	11	NULL	NULL	NULL	E2	Chemical		bind					Bmp6 gene	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_35_25509_s_17	16798745	A functional relationship between E2 and BMP-6 was further suggested by E2 binding to the  Bmp6 gene promotor ( ) and by increased BMP-6 immunostaining in bone marrow of mice treated with E2 ( ).	bind
36600	1	10288	6	NULL	NULL	0	NULL	E2	NULL		bind	NULL				Bmp6 gene	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_35_25509_s_17	16798745	A functional relationship between E2 and BMP-6 was further suggested by E2 binding to the  Bmp6 gene promotor ( ) and by increased BMP-6 immunostaining in bone marrow of mice treated with E2 ( ).	bind
43764	1	10289	5	11	NULL	NULL	NULL	Eps15	GP	human	bind			DPF repeats		AP-2	GP		alpha-adaptin subunit		NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_18_23_9638_s_315	9822725	A functional role for the DPF motif is suggested by a recent study that demonstrates that the binding of human Eps15 to the alpha-adaptin subunit of AP-2 is mediated by a portion of Eps15 that contains four of these DPF repeats (Benmerah et al., 1996  ).	bind
36601	1	10289	6	10	NULL	0	NULL	Eps15		human	bind			DPF repeats		AP-2			alpha-adaptin subunit		NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_18_23_9638_s_315	9822725	A functional role for the DPF motif is suggested by a recent study that demonstrates that the binding of human Eps15 to the alpha-adaptin subunit of AP-2 is mediated by a portion of Eps15 that contains four of these DPF repeats (Benmerah et al., 1996  ).	bind
43765	1	10290	5	11	NULL	NULL	NULL	SRP	GP		bind		tightly			RNCs	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_1_103_s_279	9436994	A functional signal sequence would be required to trigger tight binding of SRP to the RNCs (Walter  et al., 1981  ).	bind
36603	1	10290	6	10	NULL	0	NULL	SRP	NULL		bind	NULL	tightly			RNC	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_1_103_s_279	9436994	A functional signal sequence would be required to trigger tight binding of SRP to the RNCs (Walter  et al., 1981  ).	bind
43767	1	10291	5	11	NULL	NULL	NULL			functional	is present in				STAT6-binding site	I gene	GP			proximal promoter region	NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10800_s_213	10485906	A functional STAT6-binding site is present in the proximal promoter region of the I  gene, and binding of activated STAT6 to this site is essential for IL-4-induced gene expression ( 44).	bind
43768	2	10291	5	11	NULL	NULL	NULL	STAT6	GP	activated	bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10800_s_213	10485906	A functional STAT6-binding site is present in the proximal promoter region of the I  gene, and binding of activated STAT6 to this site is essential for IL-4-induced gene expression ( 44).	bind
43769	3	10291	5	11	NULL	NULL	NULL	IL-4	GP		induce					gene	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10800_s_213	10485906	A functional STAT6-binding site is present in the proximal promoter region of the I  gene, and binding of activated STAT6 to this site is essential for IL-4-induced gene expression ( 44).	bind
43770	4	10291	5	11	NULL	NULL	NULL	statement 2	GP		is essential for					statement 3	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_19_10800_s_213	10485906	A functional STAT6-binding site is present in the proximal promoter region of the I  gene, and binding of activated STAT6 to this site is essential for IL-4-induced gene expression ( 44).	bind
36604	1	10291	6	NULL	NULL	0	NULL	STAT6	NULL	activated	bind	NULL				I gene	NULL	functional		STAT6-binding site of promoter	NULL		0	NULL	NULL	NULL	gw60_pnas_96_19_10800_s_213	10485906	A functional STAT6-binding site is present in the proximal promoter region of the I  gene, and binding of activated STAT6 to this site is essential for IL-4-induced gene expression ( 44).	bind
36605	2	10291	6	NULL	NULL	0	NULL	IL-4	NULL		induces	NULL				I gene	NULL	expression of			NULL		0	NULL	NULL	NULL	gw60_pnas_96_19_10800_s_213	10485906	A functional STAT6-binding site is present in the proximal promoter region of the I  gene, and binding of activated STAT6 to this site is essential for IL-4-induced gene expression ( 44).	bind
36606	3	10291	6	NULL	NULL	0	NULL	statement 1	NULL		is essential for	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_96_19_10800_s_213	10485906	A functional STAT6-binding site is present in the proximal promoter region of the I  gene, and binding of activated STAT6 to this site is essential for IL-4-induced gene expression ( 44).	bind
43771	1	10292	5	11	NULL	NULL	NULL				bind			p40 Subunit		ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_20_11607_s_99	9751713	A Functional Walker A Motif Is Required for ATP Binding to the p40 Subunit.	bind
43772	2	10292	5	11	NULL	NULL	NULL			functional	is required for			walker a motif		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_20_11607_s_99	9751713	A Functional Walker A Motif Is Required for ATP Binding to the p40 Subunit.	bind
36607	1	10292	6	10	NULL	0	NULL	ATP			bind								p40 subunit		NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_20_11607_s_99	9751713	A Functional Walker A Motif Is Required for ATP Binding to the p40 Subunit.	bind
36608	2	10292	6	NULL	NULL	0	NULL		NULL	functional	is required for	NULL		Walker A Motif		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_20_11607_s_99	9751713	A Functional Walker A Motif Is Required for ATP Binding to the p40 Subunit.	bind
43773	1	10293	5	11	NULL	NULL	NULL	synthetic peptide	GP	functional;;discontinuous;;branched	is derived from					HIV-1 gp120	GP		C3/C4 domain		NULL		NULL	NULL	NULL	NULL	gw60_embo_16_10_2599_s_532	9184207	A functional, discontinuous HIV-1 gp120 C3/C4 domain-derived, branched, synthetic peptide that binds to CD4 and inhibits MIP-1{alpha} chemokine binding.	bind
43774	2	10293	5	11	NULL	NULL	NULL	statement 1	GP		bind					CD4	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_10_2599_s_532	9184207	A functional, discontinuous HIV-1 gp120 C3/C4 domain-derived, branched, synthetic peptide that binds to CD4 and inhibits MIP-1{alpha} chemokine binding.	bind
43775	3	10293	5	11	NULL	NULL	NULL	statement 2	GP		inhibit					MIP-1{alpha}	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_embo_16_10_2599_s_532	9184207	A functional, discontinuous HIV-1 gp120 C3/C4 domain-derived, branched, synthetic peptide that binds to CD4 and inhibits MIP-1{alpha} chemokine binding.	bind
43776	4	10293	5	11	NULL	NULL	NULL	MIP-1{alpha}	GP		is a type of					chemokine	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_10_2599_s_532	9184207	A functional, discontinuous HIV-1 gp120 C3/C4 domain-derived, branched, synthetic peptide that binds to CD4 and inhibits MIP-1{alpha} chemokine binding.	bind
37051	1	10293	6	10	NULL	0	NULL	synthetic peptide	NULL	\tfunctional;;discontinuous;;branched \t	is derived from	NULL				HIV-1 gp120	NULL		C3/C4 domain		NULL		NULL	NULL	NULL	NULL	gw60_embo_16_10_2599_s_532	9184207	A functional, discontinuous HIV-1 gp120 C3/C4 domain-derived, branched, synthetic peptide that binds to CD4 and inhibits MIP-1{alpha} chemokine binding.	bind
37052	2	10293	6	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL				CD4	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_16_10_2599_s_532	9184207	A functional, discontinuous HIV-1 gp120 C3/C4 domain-derived, branched, synthetic peptide that binds to CD4 and inhibits MIP-1{alpha} chemokine binding.	bind
37053	3	10293	6	10	NULL	0	NULL	statement 1	NULL		inhibits	NULL				MIP-1{alpha}	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw60_embo_16_10_2599_s_532	9184207	A functional, discontinuous HIV-1 gp120 C3/C4 domain-derived, branched, synthetic peptide that binds to CD4 and inhibits MIP-1{alpha} chemokine binding.	bind
48437	4	10293	6	10	NULL	0	NULL	MIP-1{alpha}	NULL		is a type of	NULL				chemokine	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_16_10_2599_s_532	9184207	A functional, discontinuous HIV-1 gp120 C3/C4 domain-derived, branched, synthetic peptide that binds to CD4 and inhibits MIP-1{alpha} chemokine binding.	bind
43777	1	10294	5	11	NULL	NULL	NULL	RFX	GP		bind		cooperative			NF-Y	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_19_0_331_s_1106	11244040	A functionally essential domain of RFX5 mediates activation of  MHC class II promoters by promoting cooperative binding between RFX and NF-Y.	bind
43778	2	10294	5	11	NULL	NULL	NULL	RFX5	GP	functional	mediate			essential domain		MHC class II	GP	activation of		promoter	NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_19_0_331_s_1106	11244040	A functionally essential domain of RFX5 mediates activation of  MHC class II promoters by promoting cooperative binding between RFX and NF-Y.	bind
43779	3	10294	5	11	NULL	NULL	NULL	RFX5	GP	functional	promotes			essential domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_19_0_331_s_1106	11244040	A functionally essential domain of RFX5 mediates activation of  MHC class II promoters by promoting cooperative binding between RFX and NF-Y.	bind
43780	4	10294	5	11	NULL	NULL	NULL	statement 3	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_19_0_331_s_1106	11244040	A functionally essential domain of RFX5 mediates activation of  MHC class II promoters by promoting cooperative binding between RFX and NF-Y.	bind
36609	1	10294	6	NULL	NULL	0	NULL	RFX	NULL		bind	NULL	cooperatively			NF-Y	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_19_0_331_s_1106	11244040	A functionally essential domain of RFX5 mediates activation of  MHC class II promoters by promoting cooperative binding between RFX and NF-Y.	bind
36611	2	10294	6	NULL	NULL	0	NULL	RFX5	NULL	functional	mediates	NULL		essential domain		MHC class II	NULL	activation of		promoter	NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_19_0_331_s_1106	11244040	A functionally essential domain of RFX5 mediates activation of  MHC class II promoters by promoting cooperative binding between RFX and NF-Y.	bind
36613	3	10294	6	NULL	NULL	0	NULL	statement 2	NULL		occurs by promoting	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_19_0_331_s_1106	11244040	A functionally essential domain of RFX5 mediates activation of  MHC class II promoters by promoting cooperative binding between RFX and NF-Y.	bind
48438	4	10294	6	10	NULL	0	NULL	statement 3	NULL		leads to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_19_0_331_s_1106	11244040	A functionally essential domain of RFX5 mediates activation of  MHC class II promoters by promoting cooperative binding between RFX and NF-Y.	bind
43781	1	10297	5	11	NULL	NULL	NULL	RAG protein	GP		bind									SEs	NULL		NULL	NULL	NULL	NULL	gw60_cell_89_1_43_s_206	9094713	A fundamental difference, therefore, appears to exist in RAG  protein binding to one versus two SEs.	bind
36616	1	10297	6	NULL	NULL	0	NULL	RAG protein	NULL		bind	NULL				SE	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_89_1_43_s_206	9094713	A fundamental difference, therefore, appears to exist in RAG  protein binding to one versus two SEs.	bind
43782	1	10298	5	11	NULL	NULL	NULL	transducin	Process		bind					rhodopsin dimers	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_18_12896_s_371	16500896	A fundamental observation gleaned from docking the three-dimensional structures of rhodopsin and transducin is that transducin binds to rhodopsin dimers in such a way that one molecule of rhodopsin binds transducin and the other serves as a docking platform ( ).	bind
37054	1	10298	6	10	NULL	0	NULL	rhodopsin dimers			bind					transducin					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_18_12896_s_371	16500896	A fundamental observation gleaned from docking the three-dimensional structures of rhodopsin and transducin is that transducin binds to rhodopsin dimers in such a way that one molecule of rhodopsin binds transducin and the other serves as a docking platform ( ).	bind
43785	1	10299	5	11	NULL	NULL	NULL	GBR-hydroxy	Chemical		is released into		slowly			bloodstream	Process				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_301_3_1190_s_204	12023554	A fundamental premise of the present study is that the effects of GBR-decanoate are mediated by a slow release of GBR-hydroxy into the bloodstream, with subsequent pseudo-irreversible binding of GBR-hydroxy to DAT sites in the brain (Lewis et al., 1999  ).	bind
43786	2	10299	5	11	NULL	NULL	NULL	GBR-decanoate	Chemical	effects of	is mediated by					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_301_3_1190_s_204	12023554	A fundamental premise of the present study is that the effects of GBR-decanoate are mediated by a slow release of GBR-hydroxy into the bloodstream, with subsequent pseudo-irreversible binding of GBR-hydroxy to DAT sites in the brain (Lewis et al., 1999  ).	bind
43787	3	10299	5	11	NULL	NULL	NULL	GBR-hydroxy	Chemical		bind		pseudo-irreversible			DAT sites	GP				NULL	brain	NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_301_3_1190_s_204	12023554	A fundamental premise of the present study is that the effects of GBR-decanoate are mediated by a slow release of GBR-hydroxy into the bloodstream, with subsequent pseudo-irreversible binding of GBR-hydroxy to DAT sites in the brain (Lewis et al., 1999  ).	bind
43788	4	10299	5	11	NULL	NULL	NULL	statement 1	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_301_3_1190_s_204	12023554	A fundamental premise of the present study is that the effects of GBR-decanoate are mediated by a slow release of GBR-hydroxy into the bloodstream, with subsequent pseudo-irreversible binding of GBR-hydroxy to DAT sites in the brain (Lewis et al., 1999  ).	bind
48566	1	10299	6	NULL	NULL	0	NULL	GBR-hydroxy	NULL		is released into	NULL	slowly			bloodstream	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_301_3_1190_s_204	12023554	A fundamental premise of the present study is that the effects of GBR-decanoate are mediated by a slow release of GBR-hydroxy into the bloodstream, with subsequent pseudo-irreversible binding of GBR-hydroxy to DAT sites in the brain (Lewis et al., 1999  ).	bind
48567	2	10299	6	10	NULL	0	NULL	GBR-hydroxy			bind		pseudo-irreversibly			DAT sites					NULL	brain	NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_301_3_1190_s_204	12023554	A fundamental premise of the present study is that the effects of GBR-decanoate are mediated by a slow release of GBR-hydroxy into the bloodstream, with subsequent pseudo-irreversible binding of GBR-hydroxy to DAT sites in the brain (Lewis et al., 1999  ).	bind
48568	3	10299	6	NULL	NULL	0	NULL	GBR-decanoate	NULL	effects of	is mediated by	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_301_3_1190_s_204	12023554	A fundamental premise of the present study is that the effects of GBR-decanoate are mediated by a slow release of GBR-hydroxy into the bloodstream, with subsequent pseudo-irreversible binding of GBR-hydroxy to DAT sites in the brain (Lewis et al., 1999  ).	bind
43814	1	10300	5	11	NULL	NULL	NULL	linker histones	GP	recognition of	is a fundamental step in					chromatin	Chromosome	assembly of;;native			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_42_25817_s_2	8824211	A fundamental step in the assembly of native chromatin is the specific recognition and binding of linker histones to the nucleoprotein subunit known as the nucleosome.	bind
43815	2	10300	5	11	NULL	NULL	NULL	linker histones	GP		bind					nucleoprotein subunit	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_42_25817_s_2	8824211	A fundamental step in the assembly of native chromatin is the specific recognition and binding of linker histones to the nucleoprotein subunit known as the nucleosome.	bind
43816	3	10300	5	11	NULL	NULL	NULL	nucleoprotein subunit	GP		is known as					nucleosome	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_42_25817_s_2	8824211	A fundamental step in the assembly of native chromatin is the specific recognition and binding of linker histones to the nucleoprotein subunit known as the nucleosome.	bind
43817	4	10300	5	11	NULL	NULL	NULL	statement 2	Process		is a fundamental step in					chromatin	Chromosome	assembly of;;native			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_42_25817_s_2	8824211	A fundamental step in the assembly of native chromatin is the specific recognition and binding of linker histones to the nucleoprotein subunit known as the nucleosome.	bind
36618	1	10300	6	NULL	NULL	0	NULL	nucleosome	NULL		is the	NULL				nucleoprotein subunit	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_42_25817_s_2	8824211	A fundamental step in the assembly of native chromatin is the specific recognition and binding of linker histones to the nucleoprotein subunit known as the nucleosome.	bind
36620	2	10300	6	NULL	NULL	0	NULL	linker histones	NULL		recognize	NULL				nucleosome	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_42_25817_s_2	8824211	A fundamental step in the assembly of native chromatin is the specific recognition and binding of linker histones to the nucleoprotein subunit known as the nucleosome.	bind
36622	3	10300	6	NULL	NULL	0	NULL	linker histones	NULL		bind	NULL				nucleosomes	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_42_25817_s_2	8824211	A fundamental step in the assembly of native chromatin is the specific recognition and binding of linker histones to the nucleoprotein subunit known as the nucleosome.	bind
36623	4	10300	6	NULL	NULL	0	NULL	statement 2	NULL		occurs simultaneously with	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_42_25817_s_2	8824211	A fundamental step in the assembly of native chromatin is the specific recognition and binding of linker histones to the nucleoprotein subunit known as the nucleosome.	bind
36625	5	10300	6	NULL	NULL	0	NULL	statement 4	NULL		is the fundamental step for	NULL				chromatin	NULL	assembly of;; native			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_42_25817_s_2	8824211	A fundamental step in the assembly of native chromatin is the specific recognition and binding of linker histones to the nucleoprotein subunit known as the nucleosome.	bind
43818	1	10301	5	11	NULL	NULL	NULL	p300	GP	highly purified	bind		strongly			GST-VP16	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_3_551_s_145	11030335	A further analysis with very highly purified p300 showed very strong binding to GST-VP16 and more moderate binding to GST-SP1 but no detectable binding to GST-CTF1 or GST alone (  Figure 7C).	bind
43819	2	10301	5	11	NULL	NULL	NULL	p300	GP	highly purified	bind		moderatley			GST-SP1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_3_551_s_145	11030335	A further analysis with very highly purified p300 showed very strong binding to GST-VP16 and more moderate binding to GST-SP1 but no detectable binding to GST-CTF1 or GST alone (  Figure 7C).	bind
43820	3	10301	5	11	NULL	NULL	NULL	p300	GP	highly purified	does not bind					GST-CTF1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_3_551_s_145	11030335	A further analysis with very highly purified p300 showed very strong binding to GST-VP16 and more moderate binding to GST-SP1 but no detectable binding to GST-CTF1 or GST alone (  Figure 7C).	bind
43821	4	10301	5	11	NULL	NULL	NULL	p300	GP	highly purified	does not bind					GST	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_3_551_s_145	11030335	A further analysis with very highly purified p300 showed very strong binding to GST-VP16 and more moderate binding to GST-SP1 but no detectable binding to GST-CTF1 or GST alone (  Figure 7C).	bind
36680	1	10301	6	NULL	NULL	0	NULL	p300	NULL	highly purified	bind	NULL	very strongly			GST-VP16	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_6_3_551_s_145	11030335	A further analysis with very highly purified p300 showed very strong binding to GST-VP16 and more moderate binding to GST-SP1 but no detectable binding to GST-CTF1 or GST alone (  Figure 7C).	bind
36681	2	10301	6	NULL	NULL	0	NULL	p300	NULL	highly purified	bind	NULL	moderately			GST-SP1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_6_3_551_s_145	11030335	A further analysis with very highly purified p300 showed very strong binding to GST-VP16 and more moderate binding to GST-SP1 but no detectable binding to GST-CTF1 or GST alone (  Figure 7C).	bind
36682	3	10301	6	NULL	NULL	0	NULL	p300	NULL	highly purified	does not bind	NULL				GST-CTF1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_6_3_551_s_145	11030335	A further analysis with very highly purified p300 showed very strong binding to GST-VP16 and more moderate binding to GST-SP1 but no detectable binding to GST-CTF1 or GST alone (  Figure 7C).	bind
36689	4	10301	6	NULL	NULL	0	NULL	p300	NULL	highly purified	does not bind	NULL				GST	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_6_3_551_s_145	11030335	A further analysis with very highly purified p300 showed very strong binding to GST-VP16 and more moderate binding to GST-SP1 but no detectable binding to GST-CTF1 or GST alone (  Figure 7C).	bind
43827	1	10302	5	11	NULL	NULL	NULL	pol delta	GP		interact with					PCNA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_27_24340_s_172	11986310	A further argument against the third subunit being the mediator of the interaction between pol delta and PCNA is the observation that deletion of the PCNA-binding motif of Pol32 in  S. cerevisiae did not significantly affect the processivity of PCNA-dependent DNA synthesis by pol delta ( 54).	bind
43828	2	10302	5	11	NULL	NULL	NULL	pol delta	GP		synthesizes					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_27_24340_s_172	11986310	A further argument against the third subunit being the mediator of the interaction between pol delta and PCNA is the observation that deletion of the PCNA-binding motif of Pol32 in  S. cerevisiae did not significantly affect the processivity of PCNA-dependent DNA synthesis by pol delta ( 54).	bind
43829	3	10302	5	11	NULL	NULL	NULL	statement 2	Process		is dependent on					PCNA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_27_24340_s_172	11986310	A further argument against the third subunit being the mediator of the interaction between pol delta and PCNA is the observation that deletion of the PCNA-binding motif of Pol32 in  S. cerevisiae did not significantly affect the processivity of PCNA-dependent DNA synthesis by pol delta ( 54).	bind
43830	4	10302	5	11	NULL	NULL	NULL	Pol32	GP	S. cerevisiae;;deletion mutant	does not affect		significantly	PCNA-binding motif		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_27_24340_s_172	11986310	A further argument against the third subunit being the mediator of the interaction between pol delta and PCNA is the observation that deletion of the PCNA-binding motif of Pol32 in  S. cerevisiae did not significantly affect the processivity of PCNA-dependent DNA synthesis by pol delta ( 54).	bind
37056	1	10302	6	NULL	NULL	0	NULL	Poldelta	NULL		synthesizes	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_27_24340_s_172	11986310	A further argument against the third subunit being the mediator of the interaction between pol delta and PCNA is the observation that deletion of the PCNA-binding motif of Pol32 in  S. cerevisiae did not significantly affect the processivity of PCNA-dependent DNA synthesis by pol delta ( 54).	bind
37057	2	10302	6	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				PCNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_27_24340_s_172	11986310	A further argument against the third subunit being the mediator of the interaction between pol delta and PCNA is the observation that deletion of the PCNA-binding motif of Pol32 in  S. cerevisiae did not significantly affect the processivity of PCNA-dependent DNA synthesis by pol delta ( 54).	bind
37058	3	10302	6	10	NULL	0	NULL	Pol32		S. cerevisiae;;deletion mutant	did not affect		significantly	PCNA-binding motif		statement 2					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_27_24340_s_172	11986310	A further argument against the third subunit being the mediator of the interaction between pol delta and PCNA is the observation that deletion of the PCNA-binding motif of Pol32 in  S. cerevisiae did not significantly affect the processivity of PCNA-dependent DNA synthesis by pol delta ( 54).	bind
48572	4	10302	6	10	NULL	0	NULL	pol delta	NULL		interacts with	NULL				PCNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_27_24340_s_172	11986310	A further argument against the third subunit being the mediator of the interaction between pol delta and PCNA is the observation that deletion of the PCNA-binding motif of Pol32 in  S. cerevisiae did not significantly affect the processivity of PCNA-dependent DNA synthesis by pol delta ( 54).	bind
43831	1	10303	5	11	NULL	NULL	NULL	FGF-2 monomer	GP		bind		covalently			heparin oligosaccharide	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24653_s_227	10816596	A further argument in favor of the bridging hypothesis rather than the FGF dimerization model, is the finding by Pye and Gallagher ( 37) that a conjugate of an FGF-2 monomer covalently bound to a heparin oligosaccharide showed mitogenic activity.	bind
43832	2	10303	5	11	NULL	NULL	NULL	FGF-2 monomer	GP	conjugate of	shows					mitogenic activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24653_s_227	10816596	A further argument in favor of the bridging hypothesis rather than the FGF dimerization model, is the finding by Pye and Gallagher ( 37) that a conjugate of an FGF-2 monomer covalently bound to a heparin oligosaccharide showed mitogenic activity.	bind
36690	1	10303	6	NULL	NULL	0	NULL	FGF-2 monomer 	NULL		bind	NULL	covalently			heparin oligosaccharide	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24653_s_227	10816596	A further argument in favor of the bridging hypothesis rather than the FGF dimerization model, is the finding by Pye and Gallagher ( 37) that a conjugate of an FGF-2 monomer covalently bound to a heparin oligosaccharide showed mitogenic activity.	bind
48573	2	10303	6	10	NULL	0	NULL	FGF-2 monomer	NULL	conjugate of	shows	NULL				mitogenic activity	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24653_s_227	10816596	A further argument in favor of the bridging hypothesis rather than the FGF dimerization model, is the finding by Pye and Gallagher ( 37) that a conjugate of an FGF-2 monomer covalently bound to a heparin oligosaccharide showed mitogenic activity.	bind
43833	1	10306	5	11	NULL	NULL	NULL	Munc13-1	GP		bind					syntaxin	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_138_7_1191_s_281	12711617	A further complication arises if it can be confirmed that Munc13-1 binding to syntaxin is not affected by phorbol esters (see Rhee  et al., 2002  , p. 131).	bind
36856	1	10306	6	NULL	NULL	0	NULL	Munc13-1	NULL		bind	NULL				syntaxin	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_138_7_1191_s_281	12711617	A further complication arises if it can be confirmed that Munc13-1 binding to syntaxin is not affected by phorbol esters (see Rhee  et al., 2002  , p. 131).	bind
43834	1	10307	5	11	NULL	NULL	NULL	p20	GP		bind					eIF4E	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_16_4798_s_245	9707439	A further conclusion from this study is that p20 binding to eIF4E involves some, but not all, of the surface residues bound by 4G-BD4EHis6.	bind
43835	2	10307	5	11	NULL	NULL	NULL	surface residues	AminoAcid		is bound by					4G-BD4EHis6	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_16_4798_s_245	9707439	A further conclusion from this study is that p20 binding to eIF4E involves some, but not all, of the surface residues bound by 4G-BD4EHis6.	bind
43836	3	10307	5	11	NULL	NULL	NULL	statement 1	Process		involves					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_16_4798_s_245	9707439	A further conclusion from this study is that p20 binding to eIF4E involves some, but not all, of the surface residues bound by 4G-BD4EHis6.	bind
36858	1	10307	6	NULL	NULL	0	NULL	p20	NULL		bind	NULL				eIF4E	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_17_16_4798_s_245	9707439	A further conclusion from this study is that p20 binding to eIF4E involves some, but not all, of the surface residues bound by 4G-BD4EHis6.	bind
36860	2	10307	6	10	NULL	0	NULL	surface residues	NULL		bind	NULL				4G-BD4EHis6	NULL				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_16_4798_s_245	9707439	A further conclusion from this study is that p20 binding to eIF4E involves some, but not all, of the surface residues bound by 4G-BD4EHis6.	bind
48574	3	10307	6	10	NULL	0	NULL	statement 1	NULL		involves	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_17_16_4798_s_245	9707439	A further conclusion from this study is that p20 binding to eIF4E involves some, but not all, of the surface residues bound by 4G-BD4EHis6.	bind
43837	2	10308	5	11	NULL	NULL	NULL	statement 1	Process		leads to					EGR1.DNA complex	NucleicAcid	prevalence of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_39_23999_s_187	8798634	A further confirmation that the prevalence of the EGR1.DNA complex was due to the higher binding affinity of EGR1 compared with TBP came from studies in which TFIIA was included.	bind
49539	1	10308	5	11	NULL	NULL	NULL	EGR1	GP	binding of	has high affinity to					TBP	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_39_23999_s_187	8798634	A further confirmation that the prevalence of the EGR1.DNA complex was due to the higher binding affinity of EGR1 compared with TBP came from studies in which TFIIA was included.	bind
37059	1	10308	6	NULL	NULL	0	NULL	EGR1	NULL	binding of	has high affinity to	NULL				TBP	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_39_23999_s_187	8798634	A further confirmation that the prevalence of the EGR1.DNA complex was due to the higher binding affinity of EGR1 compared with TBP came from studies in which TFIIA was included.	bind
49540	2	10308	6	10	NULL	0	NULL	statement 1	NULL		leads to	NULL				EGR1.DNA complex	NULL	prevalence of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_39_23999_s_187	8798634	A further confirmation that the prevalence of the EGR1.DNA complex was due to the higher binding affinity of EGR1 compared with TBP came from studies in which TFIIA was included.	bind
43838	1	10309	5	11	NULL	NULL	NULL	M-cyclin	GP		bind			N-terminus		cdk2	GP		T-loop		NULL		NULL	NULL	NULL	NULL	gw60_embo_19_12_2877_s_193	10856233	A further consequence of the position of M-cyclin bound to cdk2 is that almost half of the cdk2 T-loop is buried within the interface pincered between the N-terminus of M-cyclin and the PSTAIRE helix (Figure  2C).	bind
43840	3	10309	5	11	NULL	NULL	NULL	cdk2	GP		bind			T-loop		M-cyclin	GP		PSTAIRE helix		NULL		NULL	NULL	NULL	NULL	gw60_embo_19_12_2877_s_193	10856233	A further consequence of the position of M-cyclin bound to cdk2 is that almost half of the cdk2 T-loop is buried within the interface pincered between the N-terminus of M-cyclin and the PSTAIRE helix (Figure  2C).	bind
36861	1	10309	6	NULL	NULL	0	NULL	M-cyclin	NULL		bind	NULL		N-terminus		Cdk2	NULL		T loop		NULL		NULL	NULL	NULL	NULL	gw60_embo_19_12_2877_s_193	10856233	A further consequence of the position of M-cyclin bound to cdk2 is that almost half of the cdk2 T-loop is buried within the interface pincered between the N-terminus of M-cyclin and the PSTAIRE helix (Figure  2C).	bind
36862	2	10309	6	NULL	NULL	0	NULL	M-cyclin	NULL		bind	NULL		PSTAIRE helix		Cdk2	NULL		T-loop		NULL		0	NULL	NULL	NULL	gw60_embo_19_12_2877_s_193	10856233	A further consequence of the position of M-cyclin bound to cdk2 is that almost half of the cdk2 T-loop is buried within the interface pincered between the N-terminus of M-cyclin and the PSTAIRE helix (Figure  2C).	bind
46392	1	10310	5	11	NULL	NULL	NULL	CTB	Chemical	immunoreactive	bind					GM1	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_3_1260_s_104	11854209	A further construct, pMGJ913, containing a polylinker sequence encoding 13 residues inserted into the  HincII site formed immunoreactive CTB that also bound to GM1 (not shown) and was found to be halo negative by RPIHA.	bind
36863	1	10310	6	NULL	NULL	0	NULL	CTB	NULL	immunoreactive	bind	NULL				GM1	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_3_1260_s_104	11854209	A further construct, pMGJ913, containing a polylinker sequence encoding 13 residues inserted into the  HincII site formed immunoreactive CTB that also bound to GM1 (not shown) and was found to be halo negative by RPIHA.	bind
43841	1	10312	5	11	NULL	NULL	NULL	ASF/SF2	GP		does not inhibit			RS domain		IIIa-MS2I	GP	splicing of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_12579_s_155	11801589	A further dissection of ASF/SF2 demonstrated that the ASF/SF2-RS domain did not inhibit IIIa-MS2I splicing (Fig.  5,  lanes 9-12), whereas the MS2 fusion protein encoding for ASF/SF2-RBD2 inhibited IIIa-MS2I splicing ~5-fold (Fig.  5,  lanes 5-8).	bind
43842	2	10312	5	11	NULL	NULL	NULL	MS2	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_12579_s_155	11801589	A further dissection of ASF/SF2 demonstrated that the ASF/SF2-RS domain did not inhibit IIIa-MS2I splicing (Fig.  5,  lanes 9-12), whereas the MS2 fusion protein encoding for ASF/SF2-RBD2 inhibited IIIa-MS2I splicing ~5-fold (Fig.  5,  lanes 5-8).	bind
43843	3	10312	5	11	NULL	NULL	NULL	MS2	GP		encodes					ASF/SF2-RBD2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_12579_s_155	11801589	A further dissection of ASF/SF2 demonstrated that the ASF/SF2-RS domain did not inhibit IIIa-MS2I splicing (Fig.  5,  lanes 9-12), whereas the MS2 fusion protein encoding for ASF/SF2-RBD2 inhibited IIIa-MS2I splicing ~5-fold (Fig.  5,  lanes 5-8).	bind
43844	4	10312	5	11	NULL	NULL	NULL	MS2	GP		inhibit					IIIa-MS2I	GP	splicing of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_12579_s_155	11801589	A further dissection of ASF/SF2 demonstrated that the ASF/SF2-RS domain did not inhibit IIIa-MS2I splicing (Fig.  5,  lanes 9-12), whereas the MS2 fusion protein encoding for ASF/SF2-RBD2 inhibited IIIa-MS2I splicing ~5-fold (Fig.  5,  lanes 5-8).	bind
36864	1	10312	6	10	NULL	0	NULL	ASF/SF2	NULL		did not inhibit	NULL		RS domain		IIIa-MS2I	NULL	splicing of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_12579_s_155	11801589	A further dissection of ASF/SF2 demonstrated that the ASF/SF2-RS domain did not inhibit IIIa-MS2I splicing (Fig.  5,  lanes 9-12), whereas the MS2 fusion protein encoding for ASF/SF2-RBD2 inhibited IIIa-MS2I splicing ~5-fold (Fig.  5,  lanes 5-8).	bind
36865	2	10312	6	10	NULL	0	NULL	MS2			encodes for					ASF/SF2-RBD2					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_12579_s_155	11801589	A further dissection of ASF/SF2 demonstrated that the ASF/SF2-RS domain did not inhibit IIIa-MS2I splicing (Fig.  5,  lanes 9-12), whereas the MS2 fusion protein encoding for ASF/SF2-RBD2 inhibited IIIa-MS2I splicing ~5-fold (Fig.  5,  lanes 5-8).	bind
36866	3	10312	6	NULL	NULL	0	NULL	statement 2	NULL		inhibits	NULL				IIIa-MS2I	NULL	splicing of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12579_s_155	11801589	A further dissection of ASF/SF2 demonstrated that the ASF/SF2-RS domain did not inhibit IIIa-MS2I splicing (Fig.  5,  lanes 9-12), whereas the MS2 fusion protein encoding for ASF/SF2-RBD2 inhibited IIIa-MS2I splicing ~5-fold (Fig.  5,  lanes 5-8).	bind
57489	4	10312	6	10	NULL	0	NULL	MS2			is a type of					fusion protein					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12579_s_155	11801589	A further dissection of ASF/SF2 demonstrated that the ASF/SF2-RS domain did not inhibit IIIa-MS2I splicing (Fig.  5,  lanes 9-12), whereas the MS2 fusion protein encoding for ASF/SF2-RBD2 inhibited IIIa-MS2I splicing ~5-fold (Fig.  5,  lanes 5-8).	bind
43845	1	10313	5	11	NULL	NULL	NULL	Keap1	GP		is a type of					Skp1-like BTB-adaptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_5_1579_s_254	16478980	A further downstream regulated interaction is demonstrated between the Skp1-like BTB-adaptor, Keap1, that binds its substrate, the transcription factor Nrf2, but no longer binds the Cul3 scaffold under stress conditions.	bind
43846	2	10313	5	11	NULL	NULL	NULL	Keap1	GP		bind					Nrf2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_5_1579_s_254	16478980	A further downstream regulated interaction is demonstrated between the Skp1-like BTB-adaptor, Keap1, that binds its substrate, the transcription factor Nrf2, but no longer binds the Cul3 scaffold under stress conditions.	bind
43847	3	10313	5	11	NULL	NULL	NULL	Nrf2	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_5_1579_s_254	16478980	A further downstream regulated interaction is demonstrated between the Skp1-like BTB-adaptor, Keap1, that binds its substrate, the transcription factor Nrf2, but no longer binds the Cul3 scaffold under stress conditions.	bind
43848	4	10313	5	11	NULL	NULL	NULL	Keap1	GP		does not bind					Cul3	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_5_1579_s_254	16478980	A further downstream regulated interaction is demonstrated between the Skp1-like BTB-adaptor, Keap1, that binds its substrate, the transcription factor Nrf2, but no longer binds the Cul3 scaffold under stress conditions.	bind
43849	5	10313	5	11	NULL	NULL	NULL	statement 4	Process		in the presence of					stress	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_5_1579_s_254	16478980	A further downstream regulated interaction is demonstrated between the Skp1-like BTB-adaptor, Keap1, that binds its substrate, the transcription factor Nrf2, but no longer binds the Cul3 scaffold under stress conditions.	bind
48705	6	10313	5	11	NULL	NULL	NULL	statement 2	Process		occurs under					stress	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_5_1579_s_254	16478980	A further downstream regulated interaction is demonstrated between the Skp1-like BTB-adaptor, Keap1, that binds its substrate, the transcription factor Nrf2, but no longer binds the Cul3 scaffold under stress conditions.	bind
36867	1	10313	6	NULL	NULL	0	NULL	Keap1	NULL		is a type of	NULL				Skp1-like BTB-adaptor	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_5_1579_s_254	16478980	A further downstream regulated interaction is demonstrated between the Skp1-like BTB-adaptor, Keap1, that binds its substrate, the transcription factor Nrf2, but no longer binds the Cul3 scaffold under stress conditions.	bind
36868	2	10313	6	NULL	NULL	0	NULL	Keap1	NULL		bind	NULL				Nrf2	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_5_1579_s_254	16478980	A further downstream regulated interaction is demonstrated between the Skp1-like BTB-adaptor, Keap1, that binds its substrate, the transcription factor Nrf2, but no longer binds the Cul3 scaffold under stress conditions.	bind
36869	3	10313	6	NULL	NULL	0	NULL	Nrf2	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_5_1579_s_254	16478980	A further downstream regulated interaction is demonstrated between the Skp1-like BTB-adaptor, Keap1, that binds its substrate, the transcription factor Nrf2, but no longer binds the Cul3 scaffold under stress conditions.	bind
36870	4	10313	6	NULL	NULL	0	NULL	Keap1	NULL		does not bind	NULL				Cul3 	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_5_1579_s_254	16478980	A further downstream regulated interaction is demonstrated between the Skp1-like BTB-adaptor, Keap1, that binds its substrate, the transcription factor Nrf2, but no longer binds the Cul3 scaffold under stress conditions.	bind
36871	5	10313	6	NULL	NULL	0	NULL	Cul3	NULL		is a type of	NULL				scaffold protein	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_5_1579_s_254	16478980	A further downstream regulated interaction is demonstrated between the Skp1-like BTB-adaptor, Keap1, that binds its substrate, the transcription factor Nrf2, but no longer binds the Cul3 scaffold under stress conditions.	bind
36872	6	10313	6	NULL	NULL	0	NULL	statement 2	NULL		occurs under	NULL				stress	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_5_1579_s_254	16478980	A further downstream regulated interaction is demonstrated between the Skp1-like BTB-adaptor, Keap1, that binds its substrate, the transcription factor Nrf2, but no longer binds the Cul3 scaffold under stress conditions.	bind
36873	7	10313	6	NULL	NULL	0	NULL	statement 4	NULL		occurs under	NULL				stress	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_5_1579_s_254	16478980	A further downstream regulated interaction is demonstrated between the Skp1-like BTB-adaptor, Keap1, that binds its substrate, the transcription factor Nrf2, but no longer binds the Cul3 scaffold under stress conditions.	bind
44177	1	10315	5	11	NULL	NULL	NULL	hNK1	GP	double mutant	shows			P112D;M291		Zn2+	Chemical	increased affinity for			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_58_2_263_s_72	10908293	A further increase in Zn2+ affinity was observed in the double mutants [P112D;M291]-hNK1 (Fig.  2A) and [P112H;M291]-hNK1 where Zn2+ inhibited 125I-BH-Substance P binding with  Ki values of 33  plus-or-minus  12 muM and 41  plus-or-minus  8 muM, respectively.	bind
44178	2	10315	5	11	NULL	NULL	NULL	hNK1	GP	double mutant	shows			P112H;M291		Zn2+	Chemical	increased affinity for			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_58_2_263_s_72	10908293	A further increase in Zn2+ affinity was observed in the double mutants [P112D;M291]-hNK1 (Fig.  2A) and [P112H;M291]-hNK1 where Zn2+ inhibited 125I-BH-Substance P binding with  Ki values of 33  plus-or-minus  12 muM and 41  plus-or-minus  8 muM, respectively.	bind
44179	3	10315	5	11	NULL	NULL	NULL	Zn2+	Chemical		inhibit					125I-BH-Substance P	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_58_2_263_s_72	10908293	A further increase in Zn2+ affinity was observed in the double mutants [P112D;M291]-hNK1 (Fig.  2A) and [P112H;M291]-hNK1 where Zn2+ inhibited 125I-BH-Substance P binding with  Ki values of 33  plus-or-minus  12 muM and 41  plus-or-minus  8 muM, respectively.	bind
36874	1	10315	6	NULL	NULL	0	NULL	Zn2+	NULL		inhibits	NULL				substance P	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_58_2_263_s_72	10908293	A further increase in Zn2+ affinity was observed in the double mutants [P112D;M291]-hNK1 (Fig.  2A) and [P112H;M291]-hNK1 where Zn2+ inhibited 125I-BH-Substance P binding with  Ki values of 33  plus-or-minus  12 muM and 41  plus-or-minus  8 muM, respectively.	bind
48706	2	10315	6	10	NULL	0	NULL	hNK1	NULL	double mutant	shows 	NULL		P112D;M291		Zn2+	NULL	increased affinity for			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_58_2_263_s_72	10908293	A further increase in Zn2+ affinity was observed in the double mutants [P112D;M291]-hNK1 (Fig.  2A) and [P112H;M291]-hNK1 where Zn2+ inhibited 125I-BH-Substance P binding with  Ki values of 33  plus-or-minus  12 muM and 41  plus-or-minus  8 muM, respectively.	bind
48707	3	10315	6	10	NULL	0	NULL	hNK1	NULL	double mutant	shows	NULL		P112H;M291		Zn2+	NULL	increased affinity for			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_58_2_263_s_72	10908293	A further increase in Zn2+ affinity was observed in the double mutants [P112D;M291]-hNK1 (Fig.  2A) and [P112H;M291]-hNK1 where Zn2+ inhibited 125I-BH-Substance P binding with  Ki values of 33  plus-or-minus  12 muM and 41  plus-or-minus  8 muM, respectively.	bind
43850	1	10316	5	11	NULL	NULL	NULL	Cdc24	GP		bind					Bud1	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_9_4463_s_153	9114012	A further indication of the residues that are important for binding of Cdc24 to Bud1 comes from analysis of the Bud1T35A mutant.	bind
36875	1	10316	6	NULL	NULL	0	NULL	Cdc24	NULL		bind	NULL				Bud1	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_94_9_4463_s_153	9114012	A further indication of the residues that are important for binding of Cdc24 to Bud1 comes from analysis of the Bud1T35A mutant.	bind
43851	1	10317	5	11	NULL	NULL	NULL	STAT-1	GP		bind					TNFR1-TRADD	GP				NULL		NULL	NULL	NULL	NULL	gw60_diabetes_51_6_1805_s_207	12031968	A further interaction between the two cytokines  signaling pathways ( 58) is through binding of STAT-1 to the TNFR1-TRADD signaling complex, which favors the formation of the DISC required for induction of apoptosis.	bind
43852	2	10317	5	11	NULL	NULL	NULL	TNFR1-TRADD	GP		is a type of					signaling complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_diabetes_51_6_1805_s_207	12031968	A further interaction between the two cytokines  signaling pathways ( 58) is through binding of STAT-1 to the TNFR1-TRADD signaling complex, which favors the formation of the DISC required for induction of apoptosis.	bind
43853	3	10317	5	11	NULL	NULL	NULL	statement 1	Process		favors					DISC	GP	formation of			NULL		NULL	NULL	NULL	NULL	gw60_diabetes_51_6_1805_s_207	12031968	A further interaction between the two cytokines  signaling pathways ( 58) is through binding of STAT-1 to the TNFR1-TRADD signaling complex, which favors the formation of the DISC required for induction of apoptosis.	bind
43854	4	10317	5	11	NULL	NULL	NULL	DISC	GP	formation of	is required for					apoptosis	Process	induction of			NULL		NULL	NULL	NULL	NULL	gw60_diabetes_51_6_1805_s_207	12031968	A further interaction between the two cytokines  signaling pathways ( 58) is through binding of STAT-1 to the TNFR1-TRADD signaling complex, which favors the formation of the DISC required for induction of apoptosis.	bind
36935	1	10317	6	10	NULL	0	NULL	STAT-1	NULL		bind	NULL				TNFR1-TRADD 	NULL				NULL		NULL	NULL	NULL	NULL	gw60_diabetes_51_6_1805_s_207	12031968	A further interaction between the two cytokines  signaling pathways ( 58) is through binding of STAT-1 to the TNFR1-TRADD signaling complex, which favors the formation of the DISC required for induction of apoptosis.	bind
36936	2	10317	6	NULL	NULL	0	NULL	statement 1	NULL		favours 	NULL				DISC	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_diabetes_51_6_1805_s_207	12031968	A further interaction between the two cytokines  signaling pathways ( 58) is through binding of STAT-1 to the TNFR1-TRADD signaling complex, which favors the formation of the DISC required for induction of apoptosis.	bind
36937	3	10317	6	10	NULL	0	NULL	DISC	NULL	formation of	is required for	NULL				apoptosis	NULL	induction of			NULL		NULL	NULL	NULL	NULL	gw60_diabetes_51_6_1805_s_207	12031968	A further interaction between the two cytokines  signaling pathways ( 58) is through binding of STAT-1 to the TNFR1-TRADD signaling complex, which favors the formation of the DISC required for induction of apoptosis.	bind
48708	4	10317	6	10	NULL	0	NULL	TNFR1-TRADD	NULL		is a type of	NULL				signaling complex	NULL				NULL		0	NULL	NULL	NULL	gw60_diabetes_51_6_1805_s_207	12031968	A further interaction between the two cytokines  signaling pathways ( 58) is through binding of STAT-1 to the TNFR1-TRADD signaling complex, which favors the formation of the DISC required for induction of apoptosis.	bind
43855	1	10318	5	11	NULL	NULL	NULL				interact with			Asn111					Asn295		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_7_4245_s_171	9020140	A further interesting but more speculative implication of the present study is that the interaction between Asn111 and Asn295 may be fundamental in determining the apparent peptide binding selectivity of AT1 and AT2 receptors.	bind
43856	4	10318	5	11	NULL	NULL	NULL	statement 1	Process		determines					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_7_4245_s_171	9020140	A further interesting but more speculative implication of the present study is that the interaction between Asn111 and Asn295 may be fundamental in determining the apparent peptide binding selectivity of AT1 and AT2 receptors.	bind
43857	5	10318	5	11	NULL	NULL	NULL	statement 1	Process		determines					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_7_4245_s_171	9020140	A further interesting but more speculative implication of the present study is that the interaction between Asn111 and Asn295 may be fundamental in determining the apparent peptide binding selectivity of AT1 and AT2 receptors.	bind
43858	2	10318	5	11	NULL	NULL	NULL	AT1 receptors	GP		bind		selectively			peptides	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_7_4245_s_171	9020140	A further interesting but more speculative implication of the present study is that the interaction between Asn111 and Asn295 may be fundamental in determining the apparent peptide binding selectivity of AT1 and AT2 receptors.	bind
43859	3	10318	5	11	NULL	NULL	NULL	AT2 receptors	GP		bind		selectively			peptides	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_7_4245_s_171	9020140	A further interesting but more speculative implication of the present study is that the interaction between Asn111 and Asn295 may be fundamental in determining the apparent peptide binding selectivity of AT1 and AT2 receptors.	bind
36942	1	10318	6	NULL	NULL	0	NULL		NULL		interacts with	NULL		Asn111			NULL		Asn295		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_7_4245_s_171	9020140	A further interesting but more speculative implication of the present study is that the interaction between Asn111 and Asn295 may be fundamental in determining the apparent peptide binding selectivity of AT1 and AT2 receptors.	bind
37875	2	10318	6	10	NULL	0	NULL	AT1 receptor	NULL		bind	NULL				peptide	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_7_4245_s_171	9020140	A further interesting but more speculative implication of the present study is that the interaction between Asn111 and Asn295 may be fundamental in determining the apparent peptide binding selectivity of AT1 and AT2 receptors.	bind
37876	3	10318	6	10	NULL	0	NULL	AT2 receptor	NULL		bind	NULL				peptide	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_7_4245_s_171	9020140	A further interesting but more speculative implication of the present study is that the interaction between Asn111 and Asn295 may be fundamental in determining the apparent peptide binding selectivity of AT1 and AT2 receptors.	bind
48709	4	10318	6	10	NULL	0	NULL	statement 1	NULL		determines	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_7_4245_s_171	9020140	A further interesting but more speculative implication of the present study is that the interaction between Asn111 and Asn295 may be fundamental in determining the apparent peptide binding selectivity of AT1 and AT2 receptors.	bind
48710	5	10318	6	10	NULL	0	NULL	statement 1	NULL		determines	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_7_4245_s_171	9020140	A further interesting but more speculative implication of the present study is that the interaction between Asn111 and Asn295 may be fundamental in determining the apparent peptide binding selectivity of AT1 and AT2 receptors.	bind
43860	1	10319	5	11	NULL	NULL	NULL	HIV-1	Organism		bind					Candida	Organism				NULL		NULL	NULL	NULL	NULL	gw70_femsimmunolmedmic_37_1_77_s_16	12770763	A further objective was to assess  whether HIV-1 binding to  Candida has an effect on fungal adhesion to human endo- or epithelial cells, representing  targets of mucosal or systemic infection, respectively.	bind
48721	2	10319	5	11	NULL	NULL	NULL	epithelial cells	Cell	human	are targets for					systemic infection	Process				NULL		NULL	NULL	NULL	NULL	gw70_femsimmunolmedmic_37_1_77_s_16	12770763	A further objective was to assess  whether HIV-1 binding to  Candida has an effect on fungal adhesion to human endo- or epithelial cells, representing  targets of mucosal or systemic infection, respectively.	bind
48722	3	10319	5	11	NULL	NULL	NULL	endothelial cells	Cell	human	are targets for					mucosal infection	Process				NULL		NULL	NULL	NULL	NULL	gw70_femsimmunolmedmic_37_1_77_s_16	12770763	A further objective was to assess  whether HIV-1 binding to  Candida has an effect on fungal adhesion to human endo- or epithelial cells, representing  targets of mucosal or systemic infection, respectively.	bind
36948	1	10319	6	NULL	NULL	0	NULL	HIV-1	NULL		bind	NULL				Candida	NULL				NULL		0	NULL	NULL	NULL	gw70_femsimmunolmedmic_37_1_77_s_16	12770763	A further objective was to assess  whether HIV-1 binding to  Candida has an effect on fungal adhesion to human endo- or epithelial cells, representing  targets of mucosal or systemic infection, respectively.	bind
36949	2	10319	6	NULL	NULL	0	NULL	endothelial cells	NULL	human	are targets for	NULL				mucosal infection	NULL				NULL		0	NULL	NULL	NULL	gw70_femsimmunolmedmic_37_1_77_s_16	12770763	A further objective was to assess  whether HIV-1 binding to  Candida has an effect on fungal adhesion to human endo- or epithelial cells, representing  targets of mucosal or systemic infection, respectively.	bind
36950	3	10319	6	10	NULL	0	NULL	epithelial cells		human	are targets for					systemic infection					NULL		NULL	NULL	NULL	NULL	gw70_femsimmunolmedmic_37_1_77_s_16	12770763	A further objective was to assess  whether HIV-1 binding to  Candida has an effect on fungal adhesion to human endo- or epithelial cells, representing  targets of mucosal or systemic infection, respectively.	bind
43861	1	10320	5	11	NULL	NULL	NULL	Rac	GP		bind					GTP	Chemical				NULL	platelets	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_47_39474_s_388	16195235	A further possibility is that a basal level of GTP-bound form of Rac is present in platelets and is sufficient to lead to initiation of lamellipodia formation.	bind
43862	2	10320	5	11	NULL	NULL	NULL	statement 1	Process		leads to		possibly			lamellipodia	MedicalFinding	initiation of;; formation of			NULL	platelets	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_47_39474_s_388	16195235	A further possibility is that a basal level of GTP-bound form of Rac is present in platelets and is sufficient to lead to initiation of lamellipodia formation.	bind
37112	1	10320	6	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				Rac	NULL				NULL	platelets	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_47_39474_s_388	16195235	A further possibility is that a basal level of GTP-bound form of Rac is present in platelets and is sufficient to lead to initiation of lamellipodia formation.	bind
37113	2	10320	6	10	NULL	0	NULL	statement 1			leads to		possibly			lamellipodia		initiation of;; formation of 			NULL	platelets	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_47_39474_s_388	16195235	A further possibility is that a basal level of GTP-bound form of Rac is present in platelets and is sufficient to lead to initiation of lamellipodia formation.	bind
43864	1	10321	5	11	NULL	NULL	NULL	LAP2	GP		bind					BAF	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_7_1754_s_287	11285238	A further prediction from our work is that the stoichiometry of LAP2 - BAF complexes varies as a function of the LAP2 concentration, and that binding between LAP2 and BAF might not follow simple first-order kinetics.	bind
37114	1	10321	6	NULL	NULL	0	NULL	LAP2	NULL		bind	NULL				BAF	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_20_7_1754_s_287	11285238	A further prediction from our work is that the stoichiometry of LAP2 - BAF complexes varies as a function of the LAP2 concentration, and that binding between LAP2 and BAF might not follow simple first-order kinetics.	bind
43866	1	10323	5	11	NULL	NULL	NULL	VCAM-1	GP		promotes		potentially			inflammation	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_42_30041_s_317	10514490	A further recent study suggested an important role for VCAM-1 in promoting inflammation in asthma by demonstrating that inhibition of binding of VCAM-1 to its ligand VLA-4 markedly inhibited lymphocyte and eosinophil infiltration in an animal model of allergen-induced inflammation ( 30).	bind
43867	2	10323	5	11	NULL	NULL	NULL	VCAM-1	GP		bind					VLA-4 ligand	GP				NULL	animal model of allergen-induced inflammation	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_42_30041_s_317	10514490	A further recent study suggested an important role for VCAM-1 in promoting inflammation in asthma by demonstrating that inhibition of binding of VCAM-1 to its ligand VLA-4 markedly inhibited lymphocyte and eosinophil infiltration in an animal model of allergen-induced inflammation ( 30).	bind
43868	3	10323	5	11	NULL	NULL	NULL	statement 1	Process		occurs during					asthma	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_42_30041_s_317	10514490	A further recent study suggested an important role for VCAM-1 in promoting inflammation in asthma by demonstrating that inhibition of binding of VCAM-1 to its ligand VLA-4 markedly inhibited lymphocyte and eosinophil infiltration in an animal model of allergen-induced inflammation ( 30).	bind
43869	4	10323	5	11	NULL	NULL	NULL	statement 2	Process	inhibition of	inhibit					lymphocyte	Cell	infiltration of			NULL	animal model of allergen-induced inflammation	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_42_30041_s_317	10514490	A further recent study suggested an important role for VCAM-1 in promoting inflammation in asthma by demonstrating that inhibition of binding of VCAM-1 to its ligand VLA-4 markedly inhibited lymphocyte and eosinophil infiltration in an animal model of allergen-induced inflammation ( 30).	bind
43870	5	10323	5	11	NULL	NULL	NULL	statement 2	Process	inhibition of	inhibit					eosinophil	Cell	infiltration of			NULL	animal model of allergen-induced inflammation	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_42_30041_s_317	10514490	A further recent study suggested an important role for VCAM-1 in promoting inflammation in asthma by demonstrating that inhibition of binding of VCAM-1 to its ligand VLA-4 markedly inhibited lymphocyte and eosinophil infiltration in an animal model of allergen-induced inflammation ( 30).	bind
37118	1	10323	6	10	NULL	0	NULL	VCAM-1			bind					VLA-4 ligand					NULL	\tanimal model of allergen-induced inflammation	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_42_30041_s_317	10514490	A further recent study suggested an important role for VCAM-1 in promoting inflammation in asthma by demonstrating that inhibition of binding of VCAM-1 to its ligand VLA-4 markedly inhibited lymphocyte and eosinophil infiltration in an animal model of allergen-induced inflammation ( 30).	bind
37119	2	10323	6	NULL	NULL	0	NULL	VCAM-1	NULL		promotes	NULL				inflammation	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_42_30041_s_317	10514490	A further recent study suggested an important role for VCAM-1 in promoting inflammation in asthma by demonstrating that inhibition of binding of VCAM-1 to its ligand VLA-4 markedly inhibited lymphocyte and eosinophil infiltration in an animal model of allergen-induced inflammation ( 30).	bind
37120	3	10323	6	NULL	NULL	0	NULL	statement 2	NULL		occurs during	NULL				Asthma	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_42_30041_s_317	10514490	A further recent study suggested an important role for VCAM-1 in promoting inflammation in asthma by demonstrating that inhibition of binding of VCAM-1 to its ligand VLA-4 markedly inhibited lymphocyte and eosinophil infiltration in an animal model of allergen-induced inflammation ( 30).	bind
37121	4	10323	6	NULL	NULL	0	NULL	statement 1	NULL	inhibition of	inhibits	NULL				lymphocyte	NULL	infiltration of			NULL	animal model of allergen-induced inflammation	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_42_30041_s_317	10514490	A further recent study suggested an important role for VCAM-1 in promoting inflammation in asthma by demonstrating that inhibition of binding of VCAM-1 to its ligand VLA-4 markedly inhibited lymphocyte and eosinophil infiltration in an animal model of allergen-induced inflammation ( 30).	bind
37122	5	10323	6	NULL	NULL	0	NULL	statement 1	NULL	inhibition of	inhibits	NULL				eosinophil	NULL	infiltration of 			NULL	animal model of allergen-induced inflammation	0	NULL	NULL	NULL	gw60_jbiolchem_274_42_30041_s_317	10514490	A further recent study suggested an important role for VCAM-1 in promoting inflammation in asthma by demonstrating that inhibition of binding of VCAM-1 to its ligand VLA-4 markedly inhibited lymphocyte and eosinophil infiltration in an animal model of allergen-induced inflammation ( 30).	bind
43871	1	10324	5	11	NULL	NULL	NULL	PLA2R	GP		bind					PLA2	GP	nonglycosylated forms of 			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_13_8780_s_53	16452473	A further relevant feature of this family of receptors is that some of them interact with other proteins through their CTLD in a sugar independent fashion, as it is the case for PLA2R that binds nonglycosylated forms of PLA2 ( ).	bind
37123	1	10324	6	NULL	NULL	0	NULL	PLA2R	NULL		bind	NULL				PLA2	NULL	nonglycosylated			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_13_8780_s_53	16452473	A further relevant feature of this family of receptors is that some of them interact with other proteins through their CTLD in a sugar independent fashion, as it is the case for PLA2R that binds nonglycosylated forms of PLA2 ( ).	bind
43877	1	10325	5	11	NULL	NULL	NULL	synthetic peptide	AminoAcid		is derived from			1399 - 1410		LN-1	GP	murine	LG4		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_45_44168_s_28	12947106	A further report shows binding of syndecan-1 from human submandibular gland cells and mouse melanoma cells B16F10 to a synthetic peptide corresponding to residues 1399 - 1410 derived from the LG4 sequence of murine LN-1 and LN-2 ( ).	bind
43878	2	10325	5	11	NULL	NULL	NULL	synthetic peptide	AminoAcid		is derived from			1399 - 1410		LN-2	GP	murine	LG4		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_45_44168_s_28	12947106	A further report shows binding of syndecan-1 from human submandibular gland cells and mouse melanoma cells B16F10 to a synthetic peptide corresponding to residues 1399 - 1410 derived from the LG4 sequence of murine LN-1 and LN-2 ( ).	bind
43879	3	10325	5	11	NULL	NULL	NULL	syndecan-1	GP	human;;submandibular gland cells	bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_45_44168_s_28	12947106	A further report shows binding of syndecan-1 from human submandibular gland cells and mouse melanoma cells B16F10 to a synthetic peptide corresponding to residues 1399 - 1410 derived from the LG4 sequence of murine LN-1 and LN-2 ( ).	bind
43880	4	10325	5	11	NULL	NULL	NULL	syndecan-1	GP	human;;submandibular gland cells	bind					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_45_44168_s_28	12947106	A further report shows binding of syndecan-1 from human submandibular gland cells and mouse melanoma cells B16F10 to a synthetic peptide corresponding to residues 1399 - 1410 derived from the LG4 sequence of murine LN-1 and LN-2 ( ).	bind
43881	5	10325	5	11	NULL	NULL	NULL	syndecan-1	GP	B16F10	bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_45_44168_s_28	12947106	A further report shows binding of syndecan-1 from human submandibular gland cells and mouse melanoma cells B16F10 to a synthetic peptide corresponding to residues 1399 - 1410 derived from the LG4 sequence of murine LN-1 and LN-2 ( ).	bind
43882	6	10325	5	11	NULL	NULL	NULL	syndecan-1	GP	B16F10	bind					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_45_44168_s_28	12947106	A further report shows binding of syndecan-1 from human submandibular gland cells and mouse melanoma cells B16F10 to a synthetic peptide corresponding to residues 1399 - 1410 derived from the LG4 sequence of murine LN-1 and LN-2 ( ).	bind
43883	7	10325	5	11	NULL	NULL	NULL	B16F10	Cell		is a type of					mouse melanoma cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_45_44168_s_28	12947106	A further report shows binding of syndecan-1 from human submandibular gland cells and mouse melanoma cells B16F10 to a synthetic peptide corresponding to residues 1399 - 1410 derived from the LG4 sequence of murine LN-1 and LN-2 ( ).	bind
37883	1	10325	6	10	NULL	0	NULL	synthetic peptide	NULL		is derived from	NULL		residues 1399 - 1410		LN-1	NULL	murine	LG4 sequence		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_45_44168_s_28	12947106	A further report shows binding of syndecan-1 from human submandibular gland cells and mouse melanoma cells B16F10 to a synthetic peptide corresponding to residues 1399 - 1410 derived from the LG4 sequence of murine LN-1 and LN-2 ( ).	bind
37884	2	10325	6	10	NULL	0	NULL	synthetic peptide	NULL		is derived from	NULL		residues 1399 - 1410		LN2	NULL	murine	LG-4 sequence		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_45_44168_s_28	12947106	A further report shows binding of syndecan-1 from human submandibular gland cells and mouse melanoma cells B16F10 to a synthetic peptide corresponding to residues 1399 - 1410 derived from the LG4 sequence of murine LN-1 and LN-2 ( ).	bind
37885	3	10325	6	10	NULL	0	NULL	syndecan-1	NULL	human;; submandibular gland cells	bind	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_45_44168_s_28	12947106	A further report shows binding of syndecan-1 from human submandibular gland cells and mouse melanoma cells B16F10 to a synthetic peptide corresponding to residues 1399 - 1410 derived from the LG4 sequence of murine LN-1 and LN-2 ( ).	bind
49562	4	10325	6	10	NULL	0	NULL	syndecan-1	NULL	human;; submandibular gland cells	bind	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_45_44168_s_28	12947106	A further report shows binding of syndecan-1 from human submandibular gland cells and mouse melanoma cells B16F10 to a synthetic peptide corresponding to residues 1399 - 1410 derived from the LG4 sequence of murine LN-1 and LN-2 ( ).	bind
49563	5	10325	6	10	NULL	0	NULL	syndecan-1	NULL	B16F10	bind	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_45_44168_s_28	12947106	A further report shows binding of syndecan-1 from human submandibular gland cells and mouse melanoma cells B16F10 to a synthetic peptide corresponding to residues 1399 - 1410 derived from the LG4 sequence of murine LN-1 and LN-2 ( ).	bind
49564	6	10325	6	10	NULL	0	NULL	syndecan-1	NULL	B16F10	bind	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_45_44168_s_28	12947106	A further report shows binding of syndecan-1 from human submandibular gland cells and mouse melanoma cells B16F10 to a synthetic peptide corresponding to residues 1399 - 1410 derived from the LG4 sequence of murine LN-1 and LN-2 ( ).	bind
49565	7	10325	6	10	NULL	0	NULL	B16F10	NULL		is a type of	NULL				mouse melanoma cells	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_45_44168_s_28	12947106	A further report shows binding of syndecan-1 from human submandibular gland cells and mouse melanoma cells B16F10 to a synthetic peptide corresponding to residues 1399 - 1410 derived from the LG4 sequence of murine LN-1 and LN-2 ( ).	bind
43884	1	10327	5	11	NULL	NULL	NULL	Rap1/Krev-1	GP		is a type of					Ras-related protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_1928_s_273	10022880	A further twist is that the Ras-related protein Rap1/Krev-1 binds to p120 Ras-GAP with high affinity but is not a substrate ( 27).	bind
43885	2	10327	5	11	NULL	NULL	NULL	Rap1/Krev-1	GP		bind		high affinity			p120 Ras-GAP	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_1928_s_273	10022880	A further twist is that the Ras-related protein Rap1/Krev-1 binds to p120 Ras-GAP with high affinity but is not a substrate ( 27).	bind
37124	1	10327	6	NULL	NULL	0	NULL	Rap1/Krev-1	NULL		bind	NULL	high affinity			p120 Ras-GAP	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_3_1928_s_273	10022880	A further twist is that the Ras-related protein Rap1/Krev-1 binds to p120 Ras-GAP with high affinity but is not a substrate ( 27).	bind
37125	2	10327	6	10	NULL	0	NULL	Rap1/Krev-1	NULL		is a type of	NULL				Ras related protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_1928_s_273	10022880	A further twist is that the Ras-related protein Rap1/Krev-1 binds to p120 Ras-GAP with high affinity but is not a substrate ( 27).	bind
43887	1	10328	5	11	NULL	NULL	NULL	LTC4	GP		bind		potentially			G protein-coupled receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_53_4_750_s_204	9547367	A further, but unlikely, hypothesis is that LTC4 binds to a G protein-coupled receptor (different from that of LTD4) but behaves as an antagonist, thus being unable to activate GTPase and displaying a GTP-insensitive binding.	bind
43888	2	10328	5	11	NULL	NULL	NULL	LTC4	GP		acts as					antagonist	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_53_4_750_s_204	9547367	A further, but unlikely, hypothesis is that LTC4 binds to a G protein-coupled receptor (different from that of LTD4) but behaves as an antagonist, thus being unable to activate GTPase and displaying a GTP-insensitive binding.	bind
43890	3	10328	5	11	NULL	NULL	NULL	LTC4	GP		does not activate					GTPase	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_53_4_750_s_204	9547367	A further, but unlikely, hypothesis is that LTC4 binds to a G protein-coupled receptor (different from that of LTD4) but behaves as an antagonist, thus being unable to activate GTPase and displaying a GTP-insensitive binding.	bind
43891	4	10328	5	11	NULL	NULL	NULL	statement 1	Process		is insensitive to					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_53_4_750_s_204	9547367	A further, but unlikely, hypothesis is that LTC4 binds to a G protein-coupled receptor (different from that of LTD4) but behaves as an antagonist, thus being unable to activate GTPase and displaying a GTP-insensitive binding.	bind
37126	1	10328	6	NULL	NULL	0	NULL	LTC4	NULL		bind	NULL				G protein-coupled receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_53_4_750_s_204	9547367	A further, but unlikely, hypothesis is that LTC4 binds to a G protein-coupled receptor (different from that of LTD4) but behaves as an antagonist, thus being unable to activate GTPase and displaying a GTP-insensitive binding.	bind
37127	2	10328	6	NULL	NULL	0	NULL	LTC4	NULL		does not activate	NULL				GTPase	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_53_4_750_s_204	9547367	A further, but unlikely, hypothesis is that LTC4 binds to a G protein-coupled receptor (different from that of LTD4) but behaves as an antagonist, thus being unable to activate GTPase and displaying a GTP-insensitive binding.	bind
37128	3	10328	6	NULL	NULL	0	NULL	LTC4	NULL		behaves as an	NULL				antagonist	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_53_4_750_s_204	9547367	A further, but unlikely, hypothesis is that LTC4 binds to a G protein-coupled receptor (different from that of LTD4) but behaves as an antagonist, thus being unable to activate GTPase and displaying a GTP-insensitive binding.	bind
37129	4	10328	6	10	NULL	0	NULL	statement 1	NULL		is insensitive to	NULL				GTP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_53_4_750_s_204	9547367	A further, but unlikely, hypothesis is that LTC4 binds to a G protein-coupled receptor (different from that of LTD4) but behaves as an antagonist, thus being unable to activate GTPase and displaying a GTP-insensitive binding.	bind
43892	1	10329	5	11	NULL	NULL	NULL				forms			N-terminal domain		thioredoxin	GP	fusion protein with			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_52_14530265_s_6	14530265	A fusion  protein of the N-terminal domain and thioredoxin binds tightly to MTs  at low salt, consistent with the increased affinity of motor domain constructs  (which contain the N-terminal domain) being due to the additional binding  of the N-terminal domain to the microtubule.	bind
43894	2	10329	5	11	NULL	NULL	NULL	statement 1	GP		bind		tightly			MTs	CellComponent				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_52_14530265_s_6	14530265	A fusion  protein of the N-terminal domain and thioredoxin binds tightly to MTs  at low salt, consistent with the increased affinity of motor domain constructs  (which contain the N-terminal domain) being due to the additional binding  of the N-terminal domain to the microtubule.	bind
43895	3	10329	5	11	NULL	NULL	NULL	statement 2	Process		in the presence of					salt	Chemical	low			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_52_14530265_s_6	14530265	A fusion  protein of the N-terminal domain and thioredoxin binds tightly to MTs  at low salt, consistent with the increased affinity of motor domain constructs  (which contain the N-terminal domain) being due to the additional binding  of the N-terminal domain to the microtubule.	bind
43901	4	10329	5	11	NULL	NULL	NULL				bind			N-terminal domain		microtubule	CellComponent				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_52_14530265_s_6	14530265	A fusion  protein of the N-terminal domain and thioredoxin binds tightly to MTs  at low salt, consistent with the increased affinity of motor domain constructs  (which contain the N-terminal domain) being due to the additional binding  of the N-terminal domain to the microtubule.	bind
37886	1	10329	6	NULL	NULL	0	NULL		NULL		forms	NULL		N-terminal domain		thioredoxin	NULL	fusion protein with			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_52_14530265_s_6	14530265	A fusion  protein of the N-terminal domain and thioredoxin binds tightly to MTs  at low salt, consistent with the increased affinity of motor domain constructs  (which contain the N-terminal domain) being due to the additional binding  of the N-terminal domain to the microtubule.	bind
37887	2	10329	6	10	NULL	0	NULL	statement 1			bind		tightly			MTs					NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_52_14530265_s_6	14530265	A fusion  protein of the N-terminal domain and thioredoxin binds tightly to MTs  at low salt, consistent with the increased affinity of motor domain constructs  (which contain the N-terminal domain) being due to the additional binding  of the N-terminal domain to the microtubule.	bind
38141	3	10329	6	NULL	NULL	0	NULL		NULL		bind	NULL		N-terminal domain		microtubule	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_52_14530265_s_6	14530265	A fusion  protein of the N-terminal domain and thioredoxin binds tightly to MTs  at low salt, consistent with the increased affinity of motor domain constructs  (which contain the N-terminal domain) being due to the additional binding  of the N-terminal domain to the microtubule.	bind
57490	4	10329	6	10	NULL	0	NULL	statement 2			in the presence of					salt		low			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_278_52_14530265_s_6	14530265	A fusion  protein of the N-terminal domain and thioredoxin binds tightly to MTs  at low salt, consistent with the increased affinity of motor domain constructs  (which contain the N-terminal domain) being due to the additional binding  of the N-terminal domain to the microtubule.	bind
43902	1	10330	5	11	NULL	NULL	NULL	GST-kendrin	GP		does not bind			coiled-coil		calmodulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_11_5919_s_72	10823944	A fusion between GST and a coiled-coil region of kendrin does not bind calmodulin, nor does GST alone.	bind
43903	2	10330	5	11	NULL	NULL	NULL	GST-kendrin	GP		is a type of			coiled-coil		fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_11_5919_s_72	10823944	A fusion between GST and a coiled-coil region of kendrin does not bind calmodulin, nor does GST alone.	bind
37130	1	10330	6	NULL	NULL	0	NULL	GST	NULL		fuses	NULL				kendrin	NULL		coiled-coil region		NULL		0	NULL	NULL	NULL	gw60_pnas_97_11_5919_s_72	10823944	A fusion between GST and a coiled-coil region of kendrin does not bind calmodulin, nor does GST alone.	bind
37131	2	10330	6	NULL	NULL	0	NULL	statement 1	NULL		does not bind	NULL				calmodulin	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_11_5919_s_72	10823944	A fusion between GST and a coiled-coil region of kendrin does not bind calmodulin, nor does GST alone.	bind
37132	3	10330	6	10	NULL	0	NULL	GST	NULL		does not bind	NULL				calmodulin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_11_5919_s_72	10823944	A fusion between GST and a coiled-coil region of kendrin does not bind calmodulin, nor does GST alone.	bind
43909	2	10340	5	11	NULL	NULL	NULL	pCTLA4-Ig	GP		contains					pCTLA4	GP	extracellular regions of			NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-immunol_165_6_10975832_s_6	10975832	A fusion protein constructed from the extracellular  regions of pCTLA4 and the constant regions of human IgG1 (pCTLA4-Ig) bound  porcine CD86 with equivalent affinity to that of hCTLA4-Ig.	bind
43910	3	10340	5	11	NULL	NULL	NULL	pCTLA4-Ig	GP		contains					IgG1	GP	human	constant regions		NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-immunol_165_6_10975832_s_6	10975832	A fusion protein constructed from the extracellular  regions of pCTLA4 and the constant regions of human IgG1 (pCTLA4-Ig) bound  porcine CD86 with equivalent affinity to that of hCTLA4-Ig.	bind
43911	1	10340	5	11	NULL	NULL	NULL	pCTLA4-Ig	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-immunol_165_6_10975832_s_6	10975832	A fusion protein constructed from the extracellular  regions of pCTLA4 and the constant regions of human IgG1 (pCTLA4-Ig) bound  porcine CD86 with equivalent affinity to that of hCTLA4-Ig.	bind
43912	4	10340	5	11	NULL	NULL	NULL	pCTLA4-Ig	GP		bind					CD86	GP	porcine			NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-immunol_165_6_10975832_s_6	10975832	A fusion protein constructed from the extracellular  regions of pCTLA4 and the constant regions of human IgG1 (pCTLA4-Ig) bound  porcine CD86 with equivalent affinity to that of hCTLA4-Ig.	bind
43913	5	10340	5	11	NULL	NULL	NULL	hCTLA4-Ig	GP		bind					CD86	GP	porcine			NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-immunol_165_6_10975832_s_6	10975832	A fusion protein constructed from the extracellular  regions of pCTLA4 and the constant regions of human IgG1 (pCTLA4-Ig) bound  porcine CD86 with equivalent affinity to that of hCTLA4-Ig.	bind
43914	6	10340	5	11	NULL	NULL	NULL	statement 4	Process		equal affinity to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-immunol_165_6_10975832_s_6	10975832	A fusion protein constructed from the extracellular  regions of pCTLA4 and the constant regions of human IgG1 (pCTLA4-Ig) bound  porcine CD86 with equivalent affinity to that of hCTLA4-Ig.	bind
37133	1	10340	6	NULL	NULL	0	NULL	pCTLA4	NULL		forms fusion protein with	NULL		extracellular region		IgG1	NULL	human	constant region		NULL		0	NULL	NULL	NULL	abs-batch0680-0699_j-immunol_165_6_10975832_s_6	10975832	A fusion protein constructed from the extracellular  regions of pCTLA4 and the constant regions of human IgG1 (pCTLA4-Ig) bound  porcine CD86 with equivalent affinity to that of hCTLA4-Ig.	bind
37134	2	10340	6	10	NULL	0	NULL	pCTLA4-Ig	NULL		bind	NULL				CD86	NULL	porcine			NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-immunol_165_6_10975832_s_6	10975832	A fusion protein constructed from the extracellular  regions of pCTLA4 and the constant regions of human IgG1 (pCTLA4-Ig) bound  porcine CD86 with equivalent affinity to that of hCTLA4-Ig.	bind
37135	3	10340	6	NULL	NULL	0	NULL	hCTLA4-Ig	NULL		bind	NULL				CD86	NULL	porcine			NULL		0	NULL	NULL	NULL	abs-batch0680-0699_j-immunol_165_6_10975832_s_6	10975832	A fusion protein constructed from the extracellular  regions of pCTLA4 and the constant regions of human IgG1 (pCTLA4-Ig) bound  porcine CD86 with equivalent affinity to that of hCTLA4-Ig.	bind
37136	4	10340	6	NULL	NULL	0	NULL	statement 2	NULL	affinity of	is equal to	NULL				statement 3	NULL	affinity of			NULL		0	NULL	NULL	NULL	abs-batch0680-0699_j-immunol_165_6_10975832_s_6	10975832	A fusion protein constructed from the extracellular  regions of pCTLA4 and the constant regions of human IgG1 (pCTLA4-Ig) bound  porcine CD86 with equivalent affinity to that of hCTLA4-Ig.	bind
57496	5	10340	6	10	NULL	0	NULL	pCTLA4-Ig			is					statement 1					NULL		0	NULL	NULL	NULL	abs-batch0680-0699_j-immunol_165_6_10975832_s_6	10975832	A fusion protein constructed from the extracellular  regions of pCTLA4 and the constant regions of human IgG1 (pCTLA4-Ig) bound  porcine CD86 with equivalent affinity to that of hCTLA4-Ig.	bind
43916	1	10341	5	11	NULL	NULL	NULL	fusion protein	GP		contains								Pro-1 region		NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-biol-chem_274_15_10187839_s_5	10187839	A fusion protein containing  the Pro-1 region showed promiscuous binding to SH3 domains of several  proteins in vitro, whereas a Pro-2 fusion bound preferentially to domains  derived from kinases.	bind
43917	2	10341	5	11	NULL	NULL	NULL	statement 1	GP		bind		promiscuous			protein	GP		SH3 domain		NULL	in vitro	NULL	NULL	NULL	NULL	abs-batch0517-0529_j-biol-chem_274_15_10187839_s_5	10187839	A fusion protein containing  the Pro-1 region showed promiscuous binding to SH3 domains of several  proteins in vitro, whereas a Pro-2 fusion bound preferentially to domains  derived from kinases.	bind
43919	3	10341	5	11	NULL	NULL	NULL	fusion protein	GP		contains								Pro-2 region		NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-biol-chem_274_15_10187839_s_5	10187839	A fusion protein containing  the Pro-1 region showed promiscuous binding to SH3 domains of several  proteins in vitro, whereas a Pro-2 fusion bound preferentially to domains  derived from kinases.	bind
43920	4	10341	5	10	NULL	0	NULL	statement 3	NULL		bind	NULL	preferentially				NULL		kinase domain		NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-biol-chem_274_15_10187839_s_5	10187839	A fusion protein containing  the Pro-1 region showed promiscuous binding to SH3 domains of several  proteins in vitro, whereas a Pro-2 fusion bound preferentially to domains  derived from kinases.	bind
37553	1	10341	6	NULL	NULL	0	NULL	Pro-1 fusion protein	NULL		bind	NULL	promiscuous				NULL		SH3 domain		NULL	in vitro	NULL	NULL	NULL	NULL	abs-batch0517-0529_j-biol-chem_274_15_10187839_s_5	10187839	A fusion protein containing  the Pro-1 region showed promiscuous binding to SH3 domains of several  proteins in vitro, whereas a Pro-2 fusion bound preferentially to domains  derived from kinases.	bind
37554	2	10341	6	10	NULL	0	NULL	Pro-2 fusion protein	NULL		bind	NULL	preferentially				NULL		kinase domain		NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-biol-chem_274_15_10187839_s_5	10187839	A fusion protein containing  the Pro-1 region showed promiscuous binding to SH3 domains of several  proteins in vitro, whereas a Pro-2 fusion bound preferentially to domains  derived from kinases.	bind
43922	1	10342	5	11	NULL	NULL	NULL	fusion protein	GP		contains					Lyn	GP		SH2 domain;;SH3 domain		NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_eur-j-immunol_27_1_9022035_s_7	9022035	A fusion protein containing Src homology 2 (SH2) and SH3 domains  of Lyn bound Syk from lysates of nonactivated RBL cells; an increased  binding was observed when lysates from Ag- or pervanadate-activated cells  were used.	bind
43924	3	10342	5	11	NULL	NULL	NULL	statement 1	GP		bind					Syk	GP				NULL	lysates of nonactivated RBL cells	NULL	NULL	NULL	NULL	abs-batch0620-0649_eur-j-immunol_27_1_9022035_s_7	9022035	A fusion protein containing Src homology 2 (SH2) and SH3 domains  of Lyn bound Syk from lysates of nonactivated RBL cells; an increased  binding was observed when lysates from Ag- or pervanadate-activated cells  were used.	bind
43927	5	10342	5	11	NULL	NULL	NULL	statement 1	GP		bind		increased			Syk	GP				NULL	lysates from Ag activated cells	NULL	NULL	NULL	NULL	abs-batch0620-0649_eur-j-immunol_27_1_9022035_s_7	9022035	A fusion protein containing Src homology 2 (SH2) and SH3 domains  of Lyn bound Syk from lysates of nonactivated RBL cells; an increased  binding was observed when lysates from Ag- or pervanadate-activated cells  were used.	bind
43929	4	10342	5	11	NULL	NULL	NULL	statement 1	GP		bind		increased			Syk	GP				NULL	lysates from pervanadate activated cells	NULL	NULL	NULL	NULL	abs-batch0620-0649_eur-j-immunol_27_1_9022035_s_7	9022035	A fusion protein containing Src homology 2 (SH2) and SH3 domains  of Lyn bound Syk from lysates of nonactivated RBL cells; an increased  binding was observed when lysates from Ag- or pervanadate-activated cells  were used.	bind
57497	2	10342	5	11	NULL	NULL	NULL	SH2	GP		is					Src homology 2	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_eur-j-immunol_27_1_9022035_s_7	9022035	A fusion protein containing Src homology 2 (SH2) and SH3 domains  of Lyn bound Syk from lysates of nonactivated RBL cells; an increased  binding was observed when lysates from Ag- or pervanadate-activated cells  were used.	bind
37624	1	10342	6	NULL	NULL	0	NULL	Src homology 2	NULL		is	NULL				SH2	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_eur-j-immunol_27_1_9022035_s_7	9022035	A fusion protein containing Src homology 2 (SH2) and SH3 domains  of Lyn bound Syk from lysates of nonactivated RBL cells; an increased  binding was observed when lysates from Ag- or pervanadate-activated cells  were used.	bind
38041	2	10342	6	10	NULL	0	NULL	Lyn			forms 			SH2 domain;;SH3 domains		fusion protein					NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_eur-j-immunol_27_1_9022035_s_7	9022035	A fusion protein containing Src homology 2 (SH2) and SH3 domains  of Lyn bound Syk from lysates of nonactivated RBL cells; an increased  binding was observed when lysates from Ag- or pervanadate-activated cells  were used.	bind
38042	3	10342	6	NULL	NULL	0	NULL	statement 2	NULL		bind	NULL				Syk	NULL				NULL	lysates of nonactivated RBL cells	0	NULL	NULL	NULL	abs-batch0620-0649_eur-j-immunol_27_1_9022035_s_7	9022035	A fusion protein containing Src homology 2 (SH2) and SH3 domains  of Lyn bound Syk from lysates of nonactivated RBL cells; an increased  binding was observed when lysates from Ag- or pervanadate-activated cells  were used.	bind
38043	4	10342	6	NULL	NULL	0	NULL	statement 2	NULL		bind	NULL				Syk	NULL				NULL	lysates from Ag- or pervanadate-activated cells	0	NULL	NULL	NULL	abs-batch0620-0649_eur-j-immunol_27_1_9022035_s_7	9022035	A fusion protein containing Src homology 2 (SH2) and SH3 domains  of Lyn bound Syk from lysates of nonactivated RBL cells; an increased  binding was observed when lysates from Ag- or pervanadate-activated cells  were used.	bind
38044	5	10342	6	NULL	NULL	0	NULL	statement 3	NULL		is greater than	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_eur-j-immunol_27_1_9022035_s_7	9022035	A fusion protein containing Src homology 2 (SH2) and SH3 domains  of Lyn bound Syk from lysates of nonactivated RBL cells; an increased  binding was observed when lysates from Ag- or pervanadate-activated cells  were used.	bind
43932	1	10344	5	11	NULL	NULL	NULL	fusion protein	GP		contains					mGluR 7A	GP		COOH-terminal		NULL		NULL	NULL	NULL	NULL	gw60_science_286_5442_1180_s_42	10550060	A fusion protein encompassing the 27 COOH-terminal amino acids of mGluR 7A (C27; see  Fig. 1A) failed to bind calmodulin, but fusion constructs N38 and N25 containing the common NH2-terminal fragments ( Fig. 1A) both bound calmodulin ( 12).	bind
43933	2	10344	5	11	NULL	NULL	NULL	statement 1	GP		does not bind					calmodulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5442_1180_s_42	10550060	A fusion protein encompassing the 27 COOH-terminal amino acids of mGluR 7A (C27; see  Fig. 1A) failed to bind calmodulin, but fusion constructs N38 and N25 containing the common NH2-terminal fragments ( Fig. 1A) both bound calmodulin ( 12).	bind
43934	3	10344	5	11	NULL	NULL	NULL	N38	GP		is a type of					fusion construct	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5442_1180_s_42	10550060	A fusion protein encompassing the 27 COOH-terminal amino acids of mGluR 7A (C27; see  Fig. 1A) failed to bind calmodulin, but fusion constructs N38 and N25 containing the common NH2-terminal fragments ( Fig. 1A) both bound calmodulin ( 12).	bind
43935	4	10344	5	11	NULL	NULL	NULL	N25	GP		is a type of					fusion construct	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5442_1180_s_42	10550060	A fusion protein encompassing the 27 COOH-terminal amino acids of mGluR 7A (C27; see  Fig. 1A) failed to bind calmodulin, but fusion constructs N38 and N25 containing the common NH2-terminal fragments ( Fig. 1A) both bound calmodulin ( 12).	bind
43936	5	10344	5	11	NULL	NULL	NULL	N38	GP		bind			N-terminal		calmodulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5442_1180_s_42	10550060	A fusion protein encompassing the 27 COOH-terminal amino acids of mGluR 7A (C27; see  Fig. 1A) failed to bind calmodulin, but fusion constructs N38 and N25 containing the common NH2-terminal fragments ( Fig. 1A) both bound calmodulin ( 12).	bind
43937	6	10344	5	11	NULL	NULL	NULL	N25	GP		bind			N-terminal		calmodulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5442_1180_s_42	10550060	A fusion protein encompassing the 27 COOH-terminal amino acids of mGluR 7A (C27; see  Fig. 1A) failed to bind calmodulin, but fusion constructs N38 and N25 containing the common NH2-terminal fragments ( Fig. 1A) both bound calmodulin ( 12).	bind
37137	1	10344	6	NULL	NULL	0	NULL	mGluR 7A	NULL		forms	NULL		COOH-terminal amino acids		fusion protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5442_1180_s_42	10550060	A fusion protein encompassing the 27 COOH-terminal amino acids of mGluR 7A (C27; see  Fig. 1A) failed to bind calmodulin, but fusion constructs N38 and N25 containing the common NH2-terminal fragments ( Fig. 1A) both bound calmodulin ( 12).	bind
38036	2	10344	6	NULL	NULL	0	NULL	statement 1	NULL		does not bind	NULL				calmodulin	NULL				NULL		0	NULL	NULL	NULL	gw60_science_286_5442_1180_s_42	10550060	A fusion protein encompassing the 27 COOH-terminal amino acids of mGluR 7A (C27; see  Fig. 1A) failed to bind calmodulin, but fusion constructs N38 and N25 containing the common NH2-terminal fragments ( Fig. 1A) both bound calmodulin ( 12).	bind
38037	3	10344	6	NULL	NULL	0	NULL	mGluR 7A	NULL		forms	NULL		NH2-terminal fragments		N38 fusion protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_science_286_5442_1180_s_42	10550060	A fusion protein encompassing the 27 COOH-terminal amino acids of mGluR 7A (C27; see  Fig. 1A) failed to bind calmodulin, but fusion constructs N38 and N25 containing the common NH2-terminal fragments ( Fig. 1A) both bound calmodulin ( 12).	bind
38038	4	10344	6	NULL	NULL	0	NULL	statement 3	NULL		bind	NULL				calmodulin	NULL				NULL		0	NULL	NULL	NULL	gw60_science_286_5442_1180_s_42	10550060	A fusion protein encompassing the 27 COOH-terminal amino acids of mGluR 7A (C27; see  Fig. 1A) failed to bind calmodulin, but fusion constructs N38 and N25 containing the common NH2-terminal fragments ( Fig. 1A) both bound calmodulin ( 12).	bind
38039	5	10344	6	NULL	NULL	0	NULL	mGluR 7A	NULL		forms	NULL		NH2-terminal fragments		N25 fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_science_286_5442_1180_s_42	10550060	A fusion protein encompassing the 27 COOH-terminal amino acids of mGluR 7A (C27; see  Fig. 1A) failed to bind calmodulin, but fusion constructs N38 and N25 containing the common NH2-terminal fragments ( Fig. 1A) both bound calmodulin ( 12).	bind
38040	6	10344	6	NULL	NULL	0	NULL	statement 5	NULL		bind	NULL				calmodulin	NULL				NULL		0	NULL	NULL	NULL	gw60_science_286_5442_1180_s_42	10550060	A fusion protein encompassing the 27 COOH-terminal amino acids of mGluR 7A (C27; see  Fig. 1A) failed to bind calmodulin, but fusion constructs N38 and N25 containing the common NH2-terminal fragments ( Fig. 1A) both bound calmodulin ( 12).	bind
44180	1	10345	5	11	NULL	NULL	NULL	fusion protein	GP		is formed by							chromosomal translocation of		t(2;13)	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_20_11719_s_104	7744814	A fusion protein formed by the t(2;13) chromosomal  translocation resulting in alveolar rhabdomyosarcoma shares DNA binding  properties with Pax3, since it includes the intact Pax3 paired and  homeodomains.	bind
44181	2	10345	5	11	NULL	NULL	NULL			chromosomal translocation of	results in				t(2;13)	alveolar rhabdomyosarcoma	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_20_11719_s_104	7744814	A fusion protein formed by the t(2;13) chromosomal  translocation resulting in alveolar rhabdomyosarcoma shares DNA binding  properties with Pax3, since it includes the intact Pax3 paired and  homeodomains.	bind
44193	3	10345	5	11	NULL	NULL	NULL	PAX3	GP		exhibits					DNA binding activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_20_11719_s_104	7744814	A fusion protein formed by the t(2;13) chromosomal  translocation resulting in alveolar rhabdomyosarcoma shares DNA binding  properties with Pax3, since it includes the intact Pax3 paired and  homeodomains.	bind
44194	4	10345	5	11	NULL	NULL	NULL	statement 1	Process		shares					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_20_11719_s_104	7744814	A fusion protein formed by the t(2;13) chromosomal  translocation resulting in alveolar rhabdomyosarcoma shares DNA binding  properties with Pax3, since it includes the intact Pax3 paired and  homeodomains.	bind
44195	5	10345	5	11	NULL	NULL	NULL	statement 1	Process		includes					Pax3	GP		paired;;homeodomain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_20_11719_s_104	7744814	A fusion protein formed by the t(2;13) chromosomal  translocation resulting in alveolar rhabdomyosarcoma shares DNA binding  properties with Pax3, since it includes the intact Pax3 paired and  homeodomains.	bind
38045	1	10345	6	10	NULL	0	NULL		NULL	chromosomal translocation of	results in	NULL			t(2;13) 	alveolar rhabdomyosarcoma	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_20_11719_s_104	7744814	A fusion protein formed by the t(2;13) chromosomal  translocation resulting in alveolar rhabdomyosarcoma shares DNA binding  properties with Pax3, since it includes the intact Pax3 paired and  homeodomains.	bind
38046	2	10345	6	10	NULL	0	NULL		NULL	chromosomal translocation of	forms	NULL			t(2;13) 	fusion protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_20_11719_s_104	7744814	A fusion protein formed by the t(2;13) chromosomal  translocation resulting in alveolar rhabdomyosarcoma shares DNA binding  properties with Pax3, since it includes the intact Pax3 paired and  homeodomains.	bind
38047	3	10345	6	10	NULL	0	NULL	statement 2			includes					Pax3			paired;;homeodomains		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_20_11719_s_104	7744814	A fusion protein formed by the t(2;13) chromosomal  translocation resulting in alveolar rhabdomyosarcoma shares DNA binding  properties with Pax3, since it includes the intact Pax3 paired and  homeodomains.	bind
38048	4	10345	6	NULL	NULL	0	NULL	Pax3	NULL		exhibits	NULL				DNA binding activity	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_20_11719_s_104	7744814	A fusion protein formed by the t(2;13) chromosomal  translocation resulting in alveolar rhabdomyosarcoma shares DNA binding  properties with Pax3, since it includes the intact Pax3 paired and  homeodomains.	bind
38049	5	10345	6	NULL	NULL	0	NULL	statement 2	NULL		shares	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_20_11719_s_104	7744814	A fusion protein formed by the t(2;13) chromosomal  translocation resulting in alveolar rhabdomyosarcoma shares DNA binding  properties with Pax3, since it includes the intact Pax3 paired and  homeodomains.	bind
43938	1	10346	5	11	NULL	NULL	NULL	pCS7299	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7293_s_194	11705900	A fusion protein lacking the last 94 amino acids of EibA (pCS7299) failed to bind IgG Fc (Fig.  5A, lane 5) and failed to form large bands, appearing instead as a monomer-sized band recognized by anti-MBP (Fig.  5B, lane 5).	bind
43939	2	10346	5	11	NULL	NULL	NULL	pCS7299	GP		lacks					EibA	GP		last 94 amino acids of		NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7293_s_194	11705900	A fusion protein lacking the last 94 amino acids of EibA (pCS7299) failed to bind IgG Fc (Fig.  5A, lane 5) and failed to form large bands, appearing instead as a monomer-sized band recognized by anti-MBP (Fig.  5B, lane 5).	bind
43940	3	10346	5	11	NULL	NULL	NULL	pCS7299	GP		does not bind					IgG Fc	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7293_s_194	11705900	A fusion protein lacking the last 94 amino acids of EibA (pCS7299) failed to bind IgG Fc (Fig.  5A, lane 5) and failed to form large bands, appearing instead as a monomer-sized band recognized by anti-MBP (Fig.  5B, lane 5).	bind
38050	1	10346	6	NULL	NULL	0	NULL	pCS7299	NULL		is a 	NULL				fusion protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7293_s_194	11705900	A fusion protein lacking the last 94 amino acids of EibA (pCS7299) failed to bind IgG Fc (Fig.  5A, lane 5) and failed to form large bands, appearing instead as a monomer-sized band recognized by anti-MBP (Fig.  5B, lane 5).	bind
38051	2	10346	6	NULL	NULL	0	NULL	statement 1	NULL		does not bind	NULL				IgG Fc	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_12_7293_s_194	11705900	A fusion protein lacking the last 94 amino acids of EibA (pCS7299) failed to bind IgG Fc (Fig.  5A, lane 5) and failed to form large bands, appearing instead as a monomer-sized band recognized by anti-MBP (Fig.  5B, lane 5).	bind
38897	3	10346	6	NULL	NULL	0	NULL	pCS7299	NULL		lacks	NULL				EibA	NULL		last 94 amino acids of		NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_12_7293_s_194	11705900	A fusion protein lacking the last 94 amino acids of EibA (pCS7299) failed to bind IgG Fc (Fig.  5A, lane 5) and failed to form large bands, appearing instead as a monomer-sized band recognized by anti-MBP (Fig.  5B, lane 5).	bind
43980	1	10347	5	11	NULL	NULL	NULL	alpha-catenin	GP		forms fusion protein with			beta-catenin-binding domain		formin-1	GP		actin polymerization domain		NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_nat-cell-biol_6_1_14647292_s_6	14647292	A fusion protein of the beta-catenin-binding  domain of alpha-catenin with the actin polymerization domains of formin-1  rescues formation of adherens junctions and associated actin cables in  alpha-catenin-null keratinocytes.	bind
43982	2	10347	5	11	NULL	NULL	NULL	statement 1	Process		rescues					adherens junctions	Cell	formation of			NULL	alpha-catenin-null keratinocytes	NULL	NULL	NULL	NULL	abs-batch0680-0699_nat-cell-biol_6_1_14647292_s_6	14647292	A fusion protein of the beta-catenin-binding  domain of alpha-catenin with the actin polymerization domains of formin-1  rescues formation of adherens junctions and associated actin cables in  alpha-catenin-null keratinocytes.	bind
43984	3	10347	5	11	NULL	NULL	NULL	statement 1	Process		rescues					actin cables	CellComponent	associated			NULL	alpha-catenin-null keratinocytes	NULL	NULL	NULL	NULL	abs-batch0680-0699_nat-cell-biol_6_1_14647292_s_6	14647292	A fusion protein of the beta-catenin-binding  domain of alpha-catenin with the actin polymerization domains of formin-1  rescues formation of adherens junctions and associated actin cables in  alpha-catenin-null keratinocytes.	bind
38052	1	10347	6	NULL	NULL	0	NULL	alpha-catenin	NULL		forms fusion protein with	NULL		beta-catenin-binding domain		formin-1	NULL		actin polymerization domain		NULL		0	NULL	NULL	NULL	abs-batch0680-0699_nat-cell-biol_6_1_14647292_s_6	14647292	A fusion protein of the beta-catenin-binding  domain of alpha-catenin with the actin polymerization domains of formin-1  rescues formation of adherens junctions and associated actin cables in  alpha-catenin-null keratinocytes.	bind
38053	2	10347	6	NULL	NULL	0	NULL	statement 1	NULL		rescues	NULL				adherens junctions	NULL	formation of			NULL	alpha-catenin-null keratinocytes	NULL	NULL	NULL	NULL	abs-batch0680-0699_nat-cell-biol_6_1_14647292_s_6	14647292	A fusion protein of the beta-catenin-binding  domain of alpha-catenin with the actin polymerization domains of formin-1  rescues formation of adherens junctions and associated actin cables in  alpha-catenin-null keratinocytes.	bind
38054	3	10347	6	NULL	NULL	0	NULL	statement 1	NULL		rescues	NULL				associated actin cables	NULL	formation of			NULL	alpha-catenin-null keratinocytes	0	NULL	NULL	NULL	abs-batch0680-0699_nat-cell-biol_6_1_14647292_s_6	14647292	A fusion protein of the beta-catenin-binding  domain of alpha-catenin with the actin polymerization domains of formin-1  rescues formation of adherens junctions and associated actin cables in  alpha-catenin-null keratinocytes.	bind
43986	1	10348	5	11	NULL	NULL	NULL	Nx1alpha-1	GP		is					neurexin Ialpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34716_s_171	9856994	A fusion protein of the entire extracellular sequence of neurexin Ialpha (Nx1alpha-1) efficiently bound neurexophilin 1 with enrichment of the processed form (Fig.  3, compare  lanes 3 and  4).	bind
43988	2	10348	5	11	NULL	NULL	NULL	Nx1alpha-1	GP		bind		efficiently	extracellular sequence		neurexophilin 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34716_s_171	9856994	A fusion protein of the entire extracellular sequence of neurexin Ialpha (Nx1alpha-1) efficiently bound neurexophilin 1 with enrichment of the processed form (Fig.  3, compare  lanes 3 and  4).	bind
37548	1	10348	6	NULL	NULL	0	NULL	neurexin Ialpha 	NULL		bind	NULL	efficiently	extracellular sequence		neurexophilin 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34716_s_171	9856994	A fusion protein of the entire extracellular sequence of neurexin Ialpha (Nx1alpha-1) efficiently bound neurexophilin 1 with enrichment of the processed form (Fig.  3, compare  lanes 3 and  4).	bind
37549	2	10348	6	NULL	NULL	0	NULL	Nx1alpha-1	NULL		is	NULL				neurexin Ialpha	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_52_34716_s_171	9856994	A fusion protein of the entire extracellular sequence of neurexin Ialpha (Nx1alpha-1) efficiently bound neurexophilin 1 with enrichment of the processed form (Fig.  3, compare  lanes 3 and  4).	bind
37550	1	10349	6	NULL	NULL	0	NULL		NULL		forms fusion protein with	NULL		N-terminal domain		thioredoxin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_52_52315_s_6	14530265	A fusion protein of the N-terminal domain and thioredoxin binds tightly to MTs at low salt, consistent with the increased affinity of motor domain constructs (which contain the N-terminal domain) being due to the additional binding of the N-terminal domain to the microtubule.	bind
37551	2	10349	6	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL	tightly			MT	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_52_52315_s_6	14530265	A fusion protein of the N-terminal domain and thioredoxin binds tightly to MTs at low salt, consistent with the increased affinity of motor domain constructs (which contain the N-terminal domain) being due to the additional binding of the N-terminal domain to the microtubule.	bind
37552	3	10349	6	NULL	NULL	0	NULL		NULL		bind	NULL		N-terminal domain		microtubule	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_52_52315_s_6	14530265	A fusion protein of the N-terminal domain and thioredoxin binds tightly to MTs at low salt, consistent with the increased affinity of motor domain constructs (which contain the N-terminal domain) being due to the additional binding of the N-terminal domain to the microtubule.	bind
43989	1	10351	5	11	NULL	NULL	NULL	Man-R	GP		is replaced with			transmembrane domain		IgG1	GP	human	constant region		NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_5_2089_s_15	9482843	A fusion protein produced by replacing the transmembrane domain of the Man-R with the constant region of human IgG1 also binds both S4GGnM-BSA and Man-BSA.	bind
43990	2	10351	5	11	NULL	NULL	NULL	statement 1	Process		forms					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_5_2089_s_15	9482843	A fusion protein produced by replacing the transmembrane domain of the Man-R with the constant region of human IgG1 also binds both S4GGnM-BSA and Man-BSA.	bind
43991	3	10351	5	11	NULL	NULL	NULL	statement 2	GP		bind					S4GGnM-BSA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_5_2089_s_15	9482843	A fusion protein produced by replacing the transmembrane domain of the Man-R with the constant region of human IgG1 also binds both S4GGnM-BSA and Man-BSA.	bind
43992	4	10351	5	11	NULL	NULL	NULL	statement 2	GP		bind					Man-BSA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_5_2089_s_15	9482843	A fusion protein produced by replacing the transmembrane domain of the Man-R with the constant region of human IgG1 also binds both S4GGnM-BSA and Man-BSA.	bind
38055	1	10351	6	NULL	NULL	0	NULL	Man-R	NULL		is replaced by	NULL		transmembrane domain		IgG1	NULL	human	constant region		NULL		0	NULL	NULL	NULL	gw60_pnas_95_5_2089_s_15	9482843	A fusion protein produced by replacing the transmembrane domain of the Man-R with the constant region of human IgG1 also binds both S4GGnM-BSA and Man-BSA.	bind
38056	2	10351	6	NULL	NULL	0	NULL	statement 1	NULL		forms a 	NULL				fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_5_2089_s_15	9482843	A fusion protein produced by replacing the transmembrane domain of the Man-R with the constant region of human IgG1 also binds both S4GGnM-BSA and Man-BSA.	bind
38057	3	10351	6	NULL	NULL	0	NULL	statement 2	NULL		bind	NULL				S4GGnM-BSA	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_5_2089_s_15	9482843	A fusion protein produced by replacing the transmembrane domain of the Man-R with the constant region of human IgG1 also binds both S4GGnM-BSA and Man-BSA.	bind
38058	4	10351	6	NULL	NULL	0	NULL	statement 2	NULL		bind	NULL				Man-BSA	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_5_2089_s_15	9482843	A fusion protein produced by replacing the transmembrane domain of the Man-R with the constant region of human IgG1 also binds both S4GGnM-BSA and Man-BSA.	bind
43993	1	10352	5	11	NULL	NULL	NULL	CaM	GP		bind					KCNQ2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_22_18_7991_s_247	12223552	A fusion protein that decreases CaM binding to KCNQ2 reduces channel activity	bind
37555	1	10352	6	NULL	NULL	0	NULL	CaM	NULL		bind	NULL				KCNQ2	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_22_18_7991_s_247	12223552	A fusion protein that decreases CaM binding to KCNQ2 reduces channel activity	bind
43996	1	10353	5	11	NULL	NULL	NULL	pDC2252	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7293_s_193	11705900	A fusion protein which retained only the last 92 amino acids of EibA (pDC2252) failed to bind IgG Fc (Fig.  5A, lane 4) but was still able to form bands larger than 200 kDa (recognized by anti-MBP) (Fig.  5B, lane 4).	bind
43997	2	10353	5	11	NULL	NULL	NULL	pDC2252	GP		retains					EibA	GP		last 92 amino acids of		NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7293_s_193	11705900	A fusion protein which retained only the last 92 amino acids of EibA (pDC2252) failed to bind IgG Fc (Fig.  5A, lane 4) but was still able to form bands larger than 200 kDa (recognized by anti-MBP) (Fig.  5B, lane 4).	bind
43998	3	10353	5	11	NULL	NULL	NULL	pDC2252	GP		does not bind					IgG Fc	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7293_s_193	11705900	A fusion protein which retained only the last 92 amino acids of EibA (pDC2252) failed to bind IgG Fc (Fig.  5A, lane 4) but was still able to form bands larger than 200 kDa (recognized by anti-MBP) (Fig.  5B, lane 4).	bind
38059	1	10353	6	10	NULL	0	NULL	pDC2252	NULL		retains	NULL				EibA	NULL		last 92 amino acids of		NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_12_7293_s_193	11705900	A fusion protein which retained only the last 92 amino acids of EibA (pDC2252) failed to bind IgG Fc (Fig.  5A, lane 4) but was still able to form bands larger than 200 kDa (recognized by anti-MBP) (Fig.  5B, lane 4).	bind
38060	2	10353	6	NULL	NULL	0	NULL	statement 1	NULL		does not bind	NULL				IgG Fc	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_12_7293_s_193	11705900	A fusion protein which retained only the last 92 amino acids of EibA (pDC2252) failed to bind IgG Fc (Fig.  5A, lane 4) but was still able to form bands larger than 200 kDa (recognized by anti-MBP) (Fig.  5B, lane 4).	bind
57498	3	10353	6	10	NULL	0	NULL	pDC2252			is a type of					fusion protein					NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_12_7293_s_193	11705900	A fusion protein which retained only the last 92 amino acids of EibA (pDC2252) failed to bind IgG Fc (Fig.  5A, lane 4) but was still able to form bands larger than 200 kDa (recognized by anti-MBP) (Fig.  5B, lane 4).	bind
43999	1	10354	5	11	NULL	NULL	NULL	amino-terminal domain	AminoAcid		is					ALCAM V2CCC Rg	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_29_17390_s_164	8663238	A fusion protein without the amino-terminal domain (ALCAM V2CCC Rg) bound very weakly to CD6 in an ELISA (Fig.  3 B), but binding to CD6 expressing cells was not detectable.	bind
44000	2	10354	5	11	NULL	NULL	NULL	fusion protein	GP	lacking	bind		weakly	amino terminal domain		CD6	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_29_17390_s_164	8663238	A fusion protein without the amino-terminal domain (ALCAM V2CCC Rg) bound very weakly to CD6 in an ELISA (Fig.  3 B), but binding to CD6 expressing cells was not detectable.	bind
38061	1	10354	6	NULL	NULL	0	NULL	fusion protein	NULL	lacking	bind	NULL	very weakly	amino-terminal domain		CD6	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_29_17390_s_164	8663238	A fusion protein without the amino-terminal domain (ALCAM V2CCC Rg) bound very weakly to CD6 in an ELISA (Fig.  3 B), but binding to CD6 expressing cells was not detectable.	bind
38062	2	10354	6	NULL	NULL	0	NULL	amino-terminal domain	NULL		is	NULL				ALCAM V2CCC Rg	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_29_17390_s_164	8663238	A fusion protein without the amino-terminal domain (ALCAM V2CCC Rg) bound very weakly to CD6 in an ELISA (Fig.  3 B), but binding to CD6 expressing cells was not detectable.	bind
44008	1	10359	5	11	NULL	NULL	NULL	RGS11	GP		bind			G protein gamma subunit-like domain					Gbeta5 subunits		NULL		NULL	NULL	NULL	NULL	gw70_annurevpharmacol_46_0_151_s_1125	16402902	A G protein  gamma subunit-like domain shared between RGS11 and other RGS proteins specifies binding  to Gbeta5 subunits.	bind
48712	2	10359	5	11	NULL	NULL	NULL	RGS proteins	GP		bind			G protein gamma subunit-like domain					Gbeta5 subunit		NULL		NULL	NULL	NULL	NULL	gw70_annurevpharmacol_46_0_151_s_1125	16402902	A G protein  gamma subunit-like domain shared between RGS11 and other RGS proteins specifies binding  to Gbeta5 subunits.	bind
38063	1	10359	6	10	NULL	0	NULL	RGS11 			bind			G protein gamma subunit-like domain					Gbeta5 subunit		NULL		NULL	NULL	NULL	NULL	gw70_annurevpharmacol_46_0_151_s_1125	16402902	A G protein  gamma subunit-like domain shared between RGS11 and other RGS proteins specifies binding  to Gbeta5 subunits.	bind
48713	2	10359	6	10	NULL	0	NULL	RGS proteins			bind			G protein gamma subunit-like domain					Gbeta5 subunit		NULL		NULL	NULL	NULL	NULL	gw70_annurevpharmacol_46_0_151_s_1125	16402902	A G protein  gamma subunit-like domain shared between RGS11 and other RGS proteins specifies binding  to Gbeta5 subunits.	bind
44011	1	10360	5	11	NULL	NULL	NULL	GTP	Chemical		bind					G protein	GP		alpha subunit		NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_5_1947_s_14	10051575	A G protein becomes activated upon the receptor-stimulated binding of GTP to its alpha subunit and continues to modulate the activity of the effector until bound GTP is hydrolyzed (reviewed in refs.	bind
44013	2	10360	5	11	NULL	NULL	NULL	receptor	GP		stimulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_5_1947_s_14	10051575	A G protein becomes activated upon the receptor-stimulated binding of GTP to its alpha subunit and continues to modulate the activity of the effector until bound GTP is hydrolyzed (reviewed in refs.	bind
44014	3	10360	5	11	NULL	NULL	NULL	statement 1	Process		activates					G protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_5_1947_s_14	10051575	A G protein becomes activated upon the receptor-stimulated binding of GTP to its alpha subunit and continues to modulate the activity of the effector until bound GTP is hydrolyzed (reviewed in refs.	bind
44015	4	10360	5	11	NULL	NULL	NULL	statement 3	Process		modulates					effector	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_5_1947_s_14	10051575	A G protein becomes activated upon the receptor-stimulated binding of GTP to its alpha subunit and continues to modulate the activity of the effector until bound GTP is hydrolyzed (reviewed in refs.	bind
44017	5	10360	5	11	NULL	NULL	NULL	statement 4	Process		occurs until					statement 1	Process	hydrolysis of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_5_1947_s_14	10051575	A G protein becomes activated upon the receptor-stimulated binding of GTP to its alpha subunit and continues to modulate the activity of the effector until bound GTP is hydrolyzed (reviewed in refs.	bind
38064	1	10360	6	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				G protein	NULL		alpha subunit		NULL		0	NULL	NULL	NULL	gw60_pnas_96_5_1947_s_14	10051575	A G protein becomes activated upon the receptor-stimulated binding of GTP to its alpha subunit and continues to modulate the activity of the effector until bound GTP is hydrolyzed (reviewed in refs.	bind
38065	2	10360	6	NULL	NULL	0	NULL	statement 1	NULL		is stimulated by	NULL				receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_96_5_1947_s_14	10051575	A G protein becomes activated upon the receptor-stimulated binding of GTP to its alpha subunit and continues to modulate the activity of the effector until bound GTP is hydrolyzed (reviewed in refs.	bind
38066	3	10360	6	NULL	NULL	0	NULL	statement 1	NULL		activates	NULL				G protein	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_96_5_1947_s_14	10051575	A G protein becomes activated upon the receptor-stimulated binding of GTP to its alpha subunit and continues to modulate the activity of the effector until bound GTP is hydrolyzed (reviewed in refs.	bind
38142	4	10360	6	NULL	NULL	0	NULL	G protein	NULL		modulates	NULL				effector	NULL	activity of 			NULL		0	NULL	NULL	NULL	gw60_pnas_96_5_1947_s_14	10051575	A G protein becomes activated upon the receptor-stimulated binding of GTP to its alpha subunit and continues to modulate the activity of the effector until bound GTP is hydrolyzed (reviewed in refs.	bind
38143	5	10360	6	NULL	NULL	0	NULL	statement 4	NULL		occurs until	NULL				statement 1	NULL	hydrolysis of			NULL		0	NULL	NULL	NULL	gw60_pnas_96_5_1947_s_14	10051575	A G protein becomes activated upon the receptor-stimulated binding of GTP to its alpha subunit and continues to modulate the activity of the effector until bound GTP is hydrolyzed (reviewed in refs.	bind
44171	1	10364	5	11	NULL	NULL	NULL	G protein	GP		uses					GTP	Chemical	binding energy of			NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_66_0_639_s_288	9242920	A G protein uses the binding energy of GTP to stabilize the switch regions to produce  a conformation that permits its association with effector.	bind
44172	2	10364	5	11	NULL	NULL	NULL	statement 1	GP		stabilize									switch regions	NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_66_0_639_s_288	9242920	A G protein uses the binding energy of GTP to stabilize the switch regions to produce  a conformation that permits its association with effector.	bind
44174	3	10364	5	11	NULL	NULL	NULL	G protein	GP		associate with					effector	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_66_0_639_s_288	9242920	A G protein uses the binding energy of GTP to stabilize the switch regions to produce  a conformation that permits its association with effector.	bind
38067	1	10364	6	NULL	NULL	0	NULL	G protein	NULL		associates with	NULL				effector	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_66_0_639_s_288	9242920	A G protein uses the binding energy of GTP to stabilize the switch regions to produce  a conformation that permits its association with effector.	bind
38130	2	10364	6	NULL	NULL	0	NULL	statement 1	NULL		uses	NULL				GTP	NULL	binding energy of 			NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_66_0_639_s_288	9242920	A G protein uses the binding energy of GTP to stabilize the switch regions to produce  a conformation that permits its association with effector.	bind
44068	1	10365	5	11	NULL	NULL	NULL	ss telomeric DNA	NucleicAcid		bind					POT1a N	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_21_5180_s_87	17053789	A G to C substitution at position 10 of the telomeric substrate abolished ss telomeric  DNA binding to both POT1a N and POT1b N, supporting previous results indicating that  this 3' terminal G10 residue is of critical importance for human POT1 binding  to telomeres (  et al).	bind
44069	2	10365	5	11	NULL	NULL	NULL	ss telomeric DNA	NucleicAcid		bind					POT1b N	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_21_5180_s_87	17053789	A G to C substitution at position 10 of the telomeric substrate abolished ss telomeric  DNA binding to both POT1a N and POT1b N, supporting previous results indicating that  this 3' terminal G10 residue is of critical importance for human POT1 binding  to telomeres (  et al).	bind
44070	3	10365	5	11	NULL	NULL	NULL	telomeric substrate	GP		is substituted to			G10		telomeric substrate	GP		C		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_21_5180_s_87	17053789	A G to C substitution at position 10 of the telomeric substrate abolished ss telomeric  DNA binding to both POT1a N and POT1b N, supporting previous results indicating that  this 3' terminal G10 residue is of critical importance for human POT1 binding  to telomeres (  et al).	bind
44071	4	10365	5	11	NULL	NULL	NULL	statement 3	Process		abolishes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_21_5180_s_87	17053789	A G to C substitution at position 10 of the telomeric substrate abolished ss telomeric  DNA binding to both POT1a N and POT1b N, supporting previous results indicating that  this 3' terminal G10 residue is of critical importance for human POT1 binding  to telomeres (  et al).	bind
44072	5	10365	5	11	NULL	NULL	NULL	statement 3	Process		abolishes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_21_5180_s_87	17053789	A G to C substitution at position 10 of the telomeric substrate abolished ss telomeric  DNA binding to both POT1a N and POT1b N, supporting previous results indicating that  this 3' terminal G10 residue is of critical importance for human POT1 binding  to telomeres (  et al).	bind
44074	6	10365	5	11	NULL	NULL	NULL	POT1	GP	human	bind					telomeres	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_21_5180_s_87	17053789	A G to C substitution at position 10 of the telomeric substrate abolished ss telomeric  DNA binding to both POT1a N and POT1b N, supporting previous results indicating that  this 3' terminal G10 residue is of critical importance for human POT1 binding  to telomeres (  et al).	bind
44075	7	10365	5	11	NULL	NULL	NULL	POT1	GP	human	is important for		critical	3' terminal G10 residue		statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_21_5180_s_87	17053789	A G to C substitution at position 10 of the telomeric substrate abolished ss telomeric  DNA binding to both POT1a N and POT1b N, supporting previous results indicating that  this 3' terminal G10 residue is of critical importance for human POT1 binding  to telomeres (  et al).	bind
38131	1	10365	6	NULL	NULL	0	NULL	ss telomeric DNA	NULL		bind	NULL				POT1a	NULL		N terminus		NULL		0	NULL	NULL	NULL	gw70_embo_25_21_5180_s_87	17053789	A G to C substitution at position 10 of the telomeric substrate abolished ss telomeric  DNA binding to both POT1a N and POT1b N, supporting previous results indicating that  this 3' terminal G10 residue is of critical importance for human POT1 binding  to telomeres (  et al).	bind
38132	2	10365	6	NULL	NULL	0	NULL	ss telomeric DNA	NULL		bind	NULL				POT1b	NULL		N terminus		NULL		0	NULL	NULL	NULL	gw70_embo_25_21_5180_s_87	17053789	A G to C substitution at position 10 of the telomeric substrate abolished ss telomeric  DNA binding to both POT1a N and POT1b N, supporting previous results indicating that  this 3' terminal G10 residue is of critical importance for human POT1 binding  to telomeres (  et al).	bind
38133	3	10365	6	NULL	NULL	0	NULL	telomeric substrate	NULL		is substituted by	NULL		G10 residue		telomeric substrate	NULL		C10 residue		NULL		0	NULL	NULL	NULL	gw70_embo_25_21_5180_s_87	17053789	A G to C substitution at position 10 of the telomeric substrate abolished ss telomeric  DNA binding to both POT1a N and POT1b N, supporting previous results indicating that  this 3' terminal G10 residue is of critical importance for human POT1 binding  to telomeres (  et al).	bind
38134	4	10365	6	NULL	NULL	0	NULL	statement 3	NULL		abolishes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_25_21_5180_s_87	17053789	A G to C substitution at position 10 of the telomeric substrate abolished ss telomeric  DNA binding to both POT1a N and POT1b N, supporting previous results indicating that  this 3' terminal G10 residue is of critical importance for human POT1 binding  to telomeres (  et al).	bind
38135	5	10365	6	NULL	NULL	0	NULL	statement 3	NULL		abolishes	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_25_21_5180_s_87	17053789	A G to C substitution at position 10 of the telomeric substrate abolished ss telomeric  DNA binding to both POT1a N and POT1b N, supporting previous results indicating that  this 3' terminal G10 residue is of critical importance for human POT1 binding  to telomeres (  et al).	bind
57499	6	10365	6	10	NULL	0	NULL	POT1		human	bind					telomeres					NULL		0	NULL	NULL	NULL	gw70_embo_25_21_5180_s_87	17053789	A G to C substitution at position 10 of the telomeric substrate abolished ss telomeric  DNA binding to both POT1a N and POT1b N, supporting previous results indicating that  this 3' terminal G10 residue is of critical importance for human POT1 binding  to telomeres (  et al).	bind
57500	7	10365	6	10	NULL	0	NULL	POT1		human	is important for		critical	3' terminal G10 residue		statement 6					NULL		0	NULL	NULL	NULL	gw70_embo_25_21_5180_s_87	17053789	A G to C substitution at position 10 of the telomeric substrate abolished ss telomeric  DNA binding to both POT1a N and POT1b N, supporting previous results indicating that  this 3' terminal G10 residue is of critical importance for human POT1 binding  to telomeres (  et al).	bind
44066	1	10366	5	11	NULL	NULL	NULL	U11	GP		bind									NRS	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_37_38201_s_133	15252020	A G-rich Downstream Element Promotes U11 Binding to the NRS --	bind
44067	2	10366	5	11	NULL	NULL	NULL				promotes				G-rich downstream element	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_37_38201_s_133	15252020	A G-rich Downstream Element Promotes U11 Binding to the NRS --	bind
38136	1	10366	6	10	NULL	0	NULL	U11			bind									NRS	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_37_38201_s_133	15252020	A G-rich Downstream Element Promotes U11 Binding to the NRS --	bind
38137	2	10366	6	NULL	NULL	0	NULL		NULL		promotes	NULL			G-rich downstream element	statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_37_38201_s_133	15252020	A G-rich Downstream Element Promotes U11 Binding to the NRS --	bind
44032	1	10368	5	11	NULL	NULL	NULL	EFTu ternary-complex	GP		bind					ribosome	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_3_460_s_612	12209000	A G-to-A mutation at base 530 reduced EFTu ternary-complex binding to the ribosome ( 156).	bind
44034	2	10368	5	11	NULL	NULL	NULL	EFTu ternary-complex	GP	mutant	reduces			G-to-A at base 530		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_3_460_s_612	12209000	A G-to-A mutation at base 530 reduced EFTu ternary-complex binding to the ribosome ( 156).	bind
38138	1	10368	6	NULL	NULL	0	NULL	EFTu ternary-complex	NULL		bind	NULL				ribosome	NULL				NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_3_460_s_612	12209000	A G-to-A mutation at base 530 reduced EFTu ternary-complex binding to the ribosome ( 156).	bind
38139	2	10368	6	NULL	NULL	0	NULL		NULL	mutant	reduces	NULL		G to A		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_3_460_s_612	12209000	A G-to-A mutation at base 530 reduced EFTu ternary-complex binding to the ribosome ( 156).	bind
44063	1	10369	5	11	NULL	NULL	NULL	trans-acting factor(s)	GP	G0 growth arrest-specific	bind					C/EBP mRNA	NucleicAcid			3''-UTR	NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_304_2_344_s_61	12711321	A G0 growth arrest-specific trans-acting factor(s) binds the C/EBP  mRNA 3''-UTR.	bind
38140	1	10369	6	10	NULL	0	NULL	trans-acting factor	NULL	G0 growth arrest-specific	bind	NULL				C/EBP mRNA	NULL			3''-UTR	NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_304_2_344_s_61	12711321	A G0 growth arrest-specific trans-acting factor(s) binds the C/EBP  mRNA 3''-UTR.	bind
44064	1	10370	5	11	NULL	NULL	NULL	G3deltaEGF	GP		is					G3 construct lacking EGF-like motifs	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_17_14178_s_27	11297534	A G3 construct lacking the EGF-like motifs (G3deltaEGF) binds to the astrocytoma cell surface.	bind
44065	2	10370	5	11	NULL	NULL	NULL	G3deltaEGF	GP		bind					astrocytoma	MedicalFinding	cell surface			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_17_14178_s_27	11297534	A G3 construct lacking the EGF-like motifs (G3deltaEGF) binds to the astrocytoma cell surface.	bind
37557	1	10370	6	10	NULL	0	NULL	G3deltaEGF	NULL		is	NULL				G3 construct lacking the EGF-like motifs	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_17_14178_s_27	11297534	A G3 construct lacking the EGF-like motifs (G3deltaEGF) binds to the astrocytoma cell surface.	bind
37558	2	10370	6	10	NULL	0	NULL	G3deltaEGF	NULL		bind	NULL				astrocytoma	NULL	cell surface			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_17_14178_s_27	11297534	A G3 construct lacking the EGF-like motifs (G3deltaEGF) binds to the astrocytoma cell surface.	bind
44077	1	10372	5	11	NULL	NULL	NULL	GATA-4	GP	deletion mutant	lacks			carboxyl-terminal					ZF1		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_8_5760_s_213	12480945	A GATA-4 carboxyl-terminal deletion mutant lacking the ZF1 and ZF2 regions did not bind RXR (Fig.  5 B).	bind
44079	2	10372	5	11	NULL	NULL	NULL	GATA-4	GP	deletion mutant	lacks			carboxyl-terminal					ZF2		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_8_5760_s_213	12480945	A GATA-4 carboxyl-terminal deletion mutant lacking the ZF1 and ZF2 regions did not bind RXR (Fig.  5 B).	bind
44080	3	10372	5	11	NULL	NULL	NULL	statement 1	GP		does not bind					RXR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_8_5760_s_213	12480945	A GATA-4 carboxyl-terminal deletion mutant lacking the ZF1 and ZF2 regions did not bind RXR (Fig.  5 B).	bind
44082	4	10372	5	11	NULL	NULL	NULL	statement 2	GP		does not bind					RXR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_8_5760_s_213	12480945	A GATA-4 carboxyl-terminal deletion mutant lacking the ZF1 and ZF2 regions did not bind RXR (Fig.  5 B).	bind
37559	1	10372	6	NULL	NULL	0	NULL	GATA-4	NULL	deletion mutant	lacks	NULL		carboxy terminal			NULL		ZF1 region		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_8_5760_s_213	12480945	A GATA-4 carboxyl-terminal deletion mutant lacking the ZF1 and ZF2 regions did not bind RXR (Fig.  5 B).	bind
37560	2	10372	6	NULL	NULL	0	NULL	GATA-4	NULL	deletion mutant	lacks	NULL		carboxyl-terminal			NULL		ZF2 region		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_8_5760_s_213	12480945	A GATA-4 carboxyl-terminal deletion mutant lacking the ZF1 and ZF2 regions did not bind RXR (Fig.  5 B).	bind
37561	3	10372	6	NULL	NULL	0	NULL	statement 1	NULL		does not bind	NULL				RXR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_8_5760_s_213	12480945	A GATA-4 carboxyl-terminal deletion mutant lacking the ZF1 and ZF2 regions did not bind RXR (Fig.  5 B).	bind
37562	4	10372	6	NULL	NULL	0	NULL	statement 2	NULL		does not bind	NULL				RXR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_8_5760_s_213	12480945	A GATA-4 carboxyl-terminal deletion mutant lacking the ZF1 and ZF2 regions did not bind RXR (Fig.  5 B).	bind
44083	1	10373	5	11	NULL	NULL	NULL	TFIIB	GP		bind					TBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_9_6260_s_23	11096089	A GC-rich sequence upstream from TATA (the BRE) can enhance TFIIB binding to the TBP.	bind
44084	2	10373	5	11	NULL	NULL	NULL	BRE	NucleicAcid		is					GC-rich sequence upstream from TATA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_9_6260_s_23	11096089	A GC-rich sequence upstream from TATA (the BRE) can enhance TFIIB binding to the TBP.	bind
44086	3	10373	5	11	NULL	NULL	NULL	TFIIB	GP		enhance				BRE	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_9_6260_s_23	11096089	A GC-rich sequence upstream from TATA (the BRE) can enhance TFIIB binding to the TBP.	bind
37563	1	10373	6	NULL	NULL	0	NULL	TFIIB	NULL		bind	NULL				TBP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_9_6260_s_23	11096089	A GC-rich sequence upstream from TATA (the BRE) can enhance TFIIB binding to the TBP.	bind
37564	2	10373	6	10	NULL	0	NULL	BRE	NULL		is	NULL				GC-rich sequence upstream from TATA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_9_6260_s_23	11096089	A GC-rich sequence upstream from TATA (the BRE) can enhance TFIIB binding to the TBP.	bind
37565	3	10373	6	10	NULL	0	NULL	TFIIB	NULL		enhance	NULL			BRE	statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_9_6260_s_23	11096089	A GC-rich sequence upstream from TATA (the BRE) can enhance TFIIB binding to the TBP.	bind
44087	1	10375	5	11	NULL	NULL	NULL	tRNA	NucleicAcid		bind								HisRS-like domains		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_16_16514_s_30	15722345	A GCN2 dimer is shown as a pair of  medium gray ribbons with tRNA bound to the HisRS-like domains.	bind
37566	1	10375	6	NULL	NULL	0	NULL	tRNA	NULL		bind	NULL					NULL		HisRS-like domain		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_16_16514_s_30	15722345	A GCN2 dimer is shown as a pair of  medium gray ribbons with tRNA bound to the HisRS-like domains.	bind
44089	1	10376	5	11	NULL	NULL	NULL	tRNA	NucleicAcid		bind								HisRS-like domains		NULL		NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_59_0_407_s_244	16153175	A Gcn2p dimer is  shown as a pair of blue ribbons with tRNA bound to the HisRS-like domains and activating  the kinase function.	bind
44090	2	10376	5	11	NULL	NULL	NULL	Gcn2p dimer	GP		activates					kinase	GP	function of			NULL		NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_59_0_407_s_244	16153175	A Gcn2p dimer is  shown as a pair of blue ribbons with tRNA bound to the HisRS-like domains and activating  the kinase function.	bind
37567	1	10376	6	NULL	NULL	0	NULL	tRNA	NULL		bind	NULL					NULL		HisRS-like domain		NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_59_0_407_s_244	16153175	A Gcn2p dimer is  shown as a pair of blue ribbons with tRNA bound to the HisRS-like domains and activating  the kinase function.	bind
37568	2	10376	6	10	NULL	0	NULL	Gcn2p dimer	NULL		activates	NULL				kinase	NULL	function of			NULL		NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_59_0_407_s_244	16153175	A Gcn2p dimer is  shown as a pair of blue ribbons with tRNA bound to the HisRS-like domains and activating  the kinase function.	bind
44092	1	10378	5	11	NULL	NULL	NULL	Rab1	GP		bind					GDP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_937_s_509	11739406	A GDP-bound form of Rab1 inhibits protein export from the endoplasmic reticulum and transport between Golgi compartments.	bind
44093	2	10378	5	11	NULL	NULL	NULL	protein	GP		is exported from					endoplasmic reticulum	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_937_s_509	11739406	A GDP-bound form of Rab1 inhibits protein export from the endoplasmic reticulum and transport between Golgi compartments.	bind
44094	3	10378	5	11	NULL	NULL	NULL	protein	GP		is transported between					Golgi compartments	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_937_s_509	11739406	A GDP-bound form of Rab1 inhibits protein export from the endoplasmic reticulum and transport between Golgi compartments.	bind
44095	4	10378	5	11	NULL	NULL	NULL	statement 1	Process		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_937_s_509	11739406	A GDP-bound form of Rab1 inhibits protein export from the endoplasmic reticulum and transport between Golgi compartments.	bind
44097	5	10378	5	11	NULL	NULL	NULL	statement 1	Process		inhibit					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_155_6_937_s_509	11739406	A GDP-bound form of Rab1 inhibits protein export from the endoplasmic reticulum and transport between Golgi compartments.	bind
37569	1	10378	6	NULL	NULL	0	NULL	GDP	NULL		bind	NULL				Rab1	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_155_6_937_s_509	11739406	A GDP-bound form of Rab1 inhibits protein export from the endoplasmic reticulum and transport between Golgi compartments.	bind
37570	2	10378	6	NULL	NULL	0	NULL	endoplasmic reticulum	NULL		exports	NULL				proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_155_6_937_s_509	11739406	A GDP-bound form of Rab1 inhibits protein export from the endoplasmic reticulum and transport between Golgi compartments.	bind
37571	3	10378	6	NULL	NULL	0	NULL	statement 1	NULL		inhibits	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_155_6_937_s_509	11739406	A GDP-bound form of Rab1 inhibits protein export from the endoplasmic reticulum and transport between Golgi compartments.	bind
37572	4	10378	6	NULL	NULL	0	NULL	protein	NULL		is transported between	NULL				golgi compartments	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_155_6_937_s_509	11739406	A GDP-bound form of Rab1 inhibits protein export from the endoplasmic reticulum and transport between Golgi compartments.	bind
37573	5	10378	6	NULL	NULL	0	NULL	statement 1	NULL		inhibits	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_155_6_937_s_509	11739406	A GDP-bound form of Rab1 inhibits protein export from the endoplasmic reticulum and transport between Golgi compartments.	bind
44099	1	10380	5	11	NULL	NULL	NULL	NAC	GP		bind					nac	GP	E. coli		promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_5_1166_s_199	9495755	A gel mobility shift assay (Fig.  5) confirms that NAC binds to the  E. coli nac promoter region, consistent with the argument that the  E. coli nac gene is autogenously regulated, just like that from  K. aerogenes.	bind
44102	2	10380	5	11	NULL	NULL	NULL	nac gene	GP	E. coli	is regulated					autogenously	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_5_1166_s_199	9495755	A gel mobility shift assay (Fig.  5) confirms that NAC binds to the  E. coli nac promoter region, consistent with the argument that the  E. coli nac gene is autogenously regulated, just like that from  K. aerogenes.	bind
44103	3	10380	5	11	NULL	NULL	NULL	nac gene	GP	K. aerogenes	is regulated					autogenously	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_5_1166_s_199	9495755	A gel mobility shift assay (Fig.  5) confirms that NAC binds to the  E. coli nac promoter region, consistent with the argument that the  E. coli nac gene is autogenously regulated, just like that from  K. aerogenes.	bind
37574	1	10380	6	10	NULL	0	NULL	NAC			bind					nac		E.coli		promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_5_1166_s_199	9495755	A gel mobility shift assay (Fig.  5) confirms that NAC binds to the  E. coli nac promoter region, consistent with the argument that the  E. coli nac gene is autogenously regulated, just like that from  K. aerogenes.	bind
37575	2	10380	6	NULL	NULL	0	NULL	statement 1	NULL		confirms	NULL				nac gene	NULL	autogeneous regulation of;; E.coli			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_5_1166_s_199	9495755	A gel mobility shift assay (Fig.  5) confirms that NAC binds to the  E. coli nac promoter region, consistent with the argument that the  E. coli nac gene is autogenously regulated, just like that from  K. aerogenes.	bind
37576	3	10380	6	NULL	NULL	0	NULL	nac gene	NULL	K. aerogenes	is 	NULL				autogenously regulated	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_5_1166_s_199	9495755	A gel mobility shift assay (Fig.  5) confirms that NAC binds to the  E. coli nac promoter region, consistent with the argument that the  E. coli nac gene is autogenously regulated, just like that from  K. aerogenes.	bind
44104	1	10381	5	11	NULL	NULL	NULL	Oct3/4	GP		bind									enhancer	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_8_2699_s_11	12665572	A gel mobility shift assay demonstrated cooperative binding of Oct3/4 and Sox2 to the enhancer sequence.	bind
44105	2	10381	5	11	NULL	NULL	NULL	Sox2	GP		bind									enhancer	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_8_2699_s_11	12665572	A gel mobility shift assay demonstrated cooperative binding of Oct3/4 and Sox2 to the enhancer sequence.	bind
57501	3	10381	5	11	NULL	NULL	NULL	statement 1	Process		occurs in cooperation with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_8_2699_s_11	12665572	A gel mobility shift assay demonstrated cooperative binding of Oct3/4 and Sox2 to the enhancer sequence.	bind
37577	1	10381	6	NULL	NULL	0	NULL	Oct3/4	NULL		bind	NULL					NULL			enhancer	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_8_2699_s_11	12665572	A gel mobility shift assay demonstrated cooperative binding of Oct3/4 and Sox2 to the enhancer sequence.	bind
37578	2	10381	6	NULL	NULL	0	NULL	Sox2	NULL		bind	NULL					NULL			enhancer	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_8_2699_s_11	12665572	A gel mobility shift assay demonstrated cooperative binding of Oct3/4 and Sox2 to the enhancer sequence.	bind
37579	3	10381	6	NULL	NULL	0	NULL	statement 1	NULL		acts in cooperation with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_8_2699_s_11	12665572	A gel mobility shift assay demonstrated cooperative binding of Oct3/4 and Sox2 to the enhancer sequence.	bind
44106	1	10382	5	11	NULL	NULL	NULL	BF-1 protein	GP	WT	bind		high affinity			S2 double-stranded oligonucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6201_s_175	10938097	A gel mobility shift assay demonstrates high-affinity binding of the WT BF-1 protein to the S2 double-stranded oligonucleotide (lane 1).	bind
37580	1	10382	6	NULL	NULL	0	NULL	BF-1 protein	NULL	wild type	bind	NULL	high affinity			S2 double-stranded oligonucleotide	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_17_6201_s_175	10938097	A gel mobility shift assay demonstrates high-affinity binding of the WT BF-1 protein to the S2 double-stranded oligonucleotide (lane 1).	bind
44107	1	10383	5	11	NULL	NULL	NULL	KKLF protein	GP	recombinant	bind					CLC-K1	GP			GA element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7319_s_8	10982849	A gel mobility shift assay revealed sequence-specific binding of recombinant KKLF and MAZ proteins to the CLC-K1 GA element, and the fine-mutation assay clarified that the consensus sequence for the KKLF binding site was GGGGNGGNG.	bind
44108	2	10383	5	11	NULL	NULL	NULL	MAZ protein	GP	recombinant	bind					CLC-K1	GP			GA element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7319_s_8	10982849	A gel mobility shift assay revealed sequence-specific binding of recombinant KKLF and MAZ proteins to the CLC-K1 GA element, and the fine-mutation assay clarified that the consensus sequence for the KKLF binding site was GGGGNGGNG.	bind
44109	3	10383	5	11	NULL	NULL	NULL	KKLF binding site	GP		is									GGGGNGGNG	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7319_s_8	10982849	A gel mobility shift assay revealed sequence-specific binding of recombinant KKLF and MAZ proteins to the CLC-K1 GA element, and the fine-mutation assay clarified that the consensus sequence for the KKLF binding site was GGGGNGGNG.	bind
37581	1	10383	6	NULL	NULL	0	NULL	KKLF protein	NULL	recombinant	bind	NULL	sequence specifically				NULL			CLC-K1GA element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7319_s_8	10982849	A gel mobility shift assay revealed sequence-specific binding of recombinant KKLF and MAZ proteins to the CLC-K1 GA element, and the fine-mutation assay clarified that the consensus sequence for the KKLF binding site was GGGGNGGNG.	bind
37582	2	10383	6	NULL	NULL	0	NULL	MAZ protein	NULL	recombinant	bind	NULL	sequence specifically				NULL			CLC-K1GA element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7319_s_8	10982849	A gel mobility shift assay revealed sequence-specific binding of recombinant KKLF and MAZ proteins to the CLC-K1 GA element, and the fine-mutation assay clarified that the consensus sequence for the KKLF binding site was GGGGNGGNG.	bind
37583	3	10383	6	10	NULL	0	NULL	KKLF binding site 			is									GGGGNGGNG	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_19_7319_s_8	10982849	A gel mobility shift assay revealed sequence-specific binding of recombinant KKLF and MAZ proteins to the CLC-K1 GA element, and the fine-mutation assay clarified that the consensus sequence for the KKLF binding site was GGGGNGGNG.	bind
44110	1	10384	5	11	NULL	NULL	NULL	protein	GP		bind					citB	GP			dyad symmetry sequence in promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_13_3304_s_214	9642180	A gel mobility shift assay showed that a protein(s) binds to the dyad symmetry sequence in the  citB promoter region ( 15).	bind
37584	1	10384	6	NULL	NULL	0	NULL	protein	NULL		bind	NULL				citB	NULL			dyad symmetry sequence of promoter	NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_13_3304_s_214	9642180	A gel mobility shift assay showed that a protein(s) binds to the dyad symmetry sequence in the  citB promoter region ( 15).	bind
44111	1	10385	5	11	NULL	NULL	NULL	Tead4 protein	GP		bind		sequence specifically							CE	NULL		NULL	NULL	NULL	NULL	gw70_development_132_21_4719_s_136	16207754	A gel mobility shift assay showed that Tead4 and Tead2 proteins bound to CE in a sequence-specific manner, as shown by competition with an excess amount of unlabeled CE oligonucleotide ( Fig. 4A, lanes 2, 3, 10, 11).	bind
44112	2	10385	5	11	NULL	NULL	NULL	Tead2 protein	GP		bind		sequence specifically							CE	NULL		NULL	NULL	NULL	NULL	gw70_development_132_21_4719_s_136	16207754	A gel mobility shift assay showed that Tead4 and Tead2 proteins bound to CE in a sequence-specific manner, as shown by competition with an excess amount of unlabeled CE oligonucleotide ( Fig. 4A, lanes 2, 3, 10, 11).	bind
48723	3	10385	5	11	NULL	NULL	NULL	CE oligonucleotide	NucleicAcid	unlabeled	bind									CE	NULL		NULL	NULL	NULL	NULL	gw70_development_132_21_4719_s_136	16207754	A gel mobility shift assay showed that Tead4 and Tead2 proteins bound to CE in a sequence-specific manner, as shown by competition with an excess amount of unlabeled CE oligonucleotide ( Fig. 4A, lanes 2, 3, 10, 11).	bind
48724	4	10385	5	11	NULL	NULL	NULL	statement 1	Process		competes with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_132_21_4719_s_136	16207754	A gel mobility shift assay showed that Tead4 and Tead2 proteins bound to CE in a sequence-specific manner, as shown by competition with an excess amount of unlabeled CE oligonucleotide ( Fig. 4A, lanes 2, 3, 10, 11).	bind
48725	5	10385	5	11	NULL	NULL	NULL	statement 2	Process		competes with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_development_132_21_4719_s_136	16207754	A gel mobility shift assay showed that Tead4 and Tead2 proteins bound to CE in a sequence-specific manner, as shown by competition with an excess amount of unlabeled CE oligonucleotide ( Fig. 4A, lanes 2, 3, 10, 11).	bind
37585	1	10385	6	NULL	NULL	0	NULL	Tead4 protein	NULL		bind	NULL	sequence specifically				NULL			CE	NULL		0	NULL	NULL	NULL	gw70_development_132_21_4719_s_136	16207754	A gel mobility shift assay showed that Tead4 and Tead2 proteins bound to CE in a sequence-specific manner, as shown by competition with an excess amount of unlabeled CE oligonucleotide ( Fig. 4A, lanes 2, 3, 10, 11).	bind
37586	2	10385	6	NULL	NULL	0	NULL	Tead2 protein	NULL		bind	NULL	sequence specifically				NULL			CE	NULL		0	NULL	NULL	NULL	gw70_development_132_21_4719_s_136	16207754	A gel mobility shift assay showed that Tead4 and Tead2 proteins bound to CE in a sequence-specific manner, as shown by competition with an excess amount of unlabeled CE oligonucleotide ( Fig. 4A, lanes 2, 3, 10, 11).	bind
37603	3	10385	6	NULL	NULL	0	NULL	CE oligonucleotide	NULL	unlabeled	bind	NULL					NULL			CE	NULL		0	NULL	NULL	NULL	gw70_development_132_21_4719_s_136	16207754	A gel mobility shift assay showed that Tead4 and Tead2 proteins bound to CE in a sequence-specific manner, as shown by competition with an excess amount of unlabeled CE oligonucleotide ( Fig. 4A, lanes 2, 3, 10, 11).	bind
37604	4	10385	6	NULL	NULL	0	NULL	statement 1	NULL		competes	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_development_132_21_4719_s_136	16207754	A gel mobility shift assay showed that Tead4 and Tead2 proteins bound to CE in a sequence-specific manner, as shown by competition with an excess amount of unlabeled CE oligonucleotide ( Fig. 4A, lanes 2, 3, 10, 11).	bind
37605	5	10385	6	NULL	NULL	0	NULL	statement 2	NULL		competes	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_development_132_21_4719_s_136	16207754	A gel mobility shift assay showed that Tead4 and Tead2 proteins bound to CE in a sequence-specific manner, as shown by competition with an excess amount of unlabeled CE oligonucleotide ( Fig. 4A, lanes 2, 3, 10, 11).	bind
44113	1	10386	5	11	NULL	NULL	NULL	NREB	GP	endogenous	bind					renin gene	GP	rat			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_9_1059_s_6	10325243	A gel mobility shift assay showed that transfected NRE TFD blocked endogenous NREB binding with the rat renin gene.	bind
44114	2	10386	5	11	NULL	NULL	NULL	NRE	GP	transfected	block			TFD		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_9_1059_s_6	10325243	A gel mobility shift assay showed that transfected NRE TFD blocked endogenous NREB binding with the rat renin gene.	bind
37606	1	10386	6	NULL	NULL	0	NULL	NREB	NULL	endogenous	bind	NULL				renin gene	NULL	rat			NULL		0	NULL	NULL	NULL	gw60_circulationres_84_9_1059_s_6	10325243	A gel mobility shift assay showed that transfected NRE TFD blocked endogenous NREB binding with the rat renin gene.	bind
37607	2	10386	6	10	NULL	0	NULL	NRE	NULL	transfected	blocks	NULL		TFD		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_9_1059_s_6	10325243	A gel mobility shift assay showed that transfected NRE TFD blocked endogenous NREB binding with the rat renin gene.	bind
44117	1	10390	5	11	NULL	NULL	NULL	U1 snRNP	GP	purified	bind					tau	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_11_4036_s_34	10805746	A gel mobility shift assay with purified U1 snRNP preparations demonstrates a significantly higher level of U1 snRNP binding to the mutant tau than to the wild-type tau pre-mRNA.	bind
44118	2	10390	5	11	NULL	NULL	NULL	U1 snRNP	GP		bind					tau pre-mRNA	NucleicAcid	wild-type			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_11_4036_s_34	10805746	A gel mobility shift assay with purified U1 snRNP preparations demonstrates a significantly higher level of U1 snRNP binding to the mutant tau than to the wild-type tau pre-mRNA.	bind
44120	3	10390	5	11	NULL	NULL	NULL	statement 1	Process		higher level than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_11_4036_s_34	10805746	A gel mobility shift assay with purified U1 snRNP preparations demonstrates a significantly higher level of U1 snRNP binding to the mutant tau than to the wild-type tau pre-mRNA.	bind
37610	1	10390	6	NULL	NULL	0	NULL	tau pre-mRNA	NULL	wild type	bind	NULL				U1 snRNP	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_11_4036_s_34	10805746	A gel mobility shift assay with purified U1 snRNP preparations demonstrates a significantly higher level of U1 snRNP binding to the mutant tau than to the wild-type tau pre-mRNA.	bind
37611	2	10390	6	NULL	NULL	0	NULL	tau pre-mRNA	NULL	mutant	bind	NULL				U1 snRNP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_11_4036_s_34	10805746	A gel mobility shift assay with purified U1 snRNP preparations demonstrates a significantly higher level of U1 snRNP binding to the mutant tau than to the wild-type tau pre-mRNA.	bind
37612	3	10390	6	NULL	NULL	0	NULL	statement 2	NULL	affinity of	is higher than	NULL				statement 1	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_11_4036_s_34	10805746	A gel mobility shift assay with purified U1 snRNP preparations demonstrates a significantly higher level of U1 snRNP binding to the mutant tau than to the wild-type tau pre-mRNA.	bind
44121	1	10393	5	11	NULL	NULL	NULL	muR1.1 RNA	NucleicAcid		bind					RNase III	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_34_13_3708_s_131	16896014	A gel shift assay ( Figure 2B) reveals that muR1.1 RNA binds RNase III to form a complex with a measured apparent dissociation constant ( ) of 205 nM ( Figure 2C).	bind
37613	1	10393	6	NULL	NULL	0	NULL	muR1.1 RNA	NULL		forms a complex with	NULL				RNase III	NULL				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_34_13_3708_s_131	16896014	A gel shift assay ( Figure 2B) reveals that muR1.1 RNA binds RNase III to form a complex with a measured apparent dissociation constant ( ) of 205 nM ( Figure 2C).	bind
44122	1	10395	5	11	NULL	NULL	NULL	ASF/SF2	GP	recombinant	bind									purine-rich element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4001_s_214	12024014	A gel shift assay performed with the purine-rich element and the CE9.7 RNA reveals that recombinant ASF/SF2 binds to the purine-rich element (Fig.  7B, lanes 2 to 5).	bind
37614	1	10395	6	NULL	NULL	0	NULL	ASF/SF2	NULL	recombinant	bind	NULL					NULL			purine-rich element	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_12_4001_s_214	12024014	A gel shift assay performed with the purine-rich element and the CE9.7 RNA reveals that recombinant ASF/SF2 binds to the purine-rich element (Fig.  7B, lanes 2 to 5).	bind
44123	1	10397	5	11	NULL	NULL	NULL	Zalpha nuclease	GP	purified	bind					Z-DNA	NucleicAcid	radioactive			NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_24_12875_s_111	9371768	A gel-mobility shift assay with a radioactive Z-DNA probe and the purified Zalpha nuclease confirms that the Zalpha nuclease binds Z-DNA with a similar affinity to that of the Zalpha domain itself (data not shown).	bind
44124	2	10397	5	11	NULL	NULL	NULL				bind			Zalpha domain		Z-DNA	NucleicAcid	radioactive			NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_24_12875_s_111	9371768	A gel-mobility shift assay with a radioactive Z-DNA probe and the purified Zalpha nuclease confirms that the Zalpha nuclease binds Z-DNA with a similar affinity to that of the Zalpha domain itself (data not shown).	bind
44125	3	10397	5	11	NULL	NULL	NULL	statement 1	Process		similar affinity to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_24_12875_s_111	9371768	A gel-mobility shift assay with a radioactive Z-DNA probe and the purified Zalpha nuclease confirms that the Zalpha nuclease binds Z-DNA with a similar affinity to that of the Zalpha domain itself (data not shown).	bind
37615	1	10397	6	10	NULL	0	NULL	Zalpha nuclease		purified	bind					Z-DNA		radioactive			NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_24_12875_s_111	9371768	A gel-mobility shift assay with a radioactive Z-DNA probe and the purified Zalpha nuclease confirms that the Zalpha nuclease binds Z-DNA with a similar affinity to that of the Zalpha domain itself (data not shown).	bind
37616	2	10397	6	NULL	NULL	0	NULL	Zalpha nuclease	NULL		bind	NULL					NULL		Zalpha domain
\n		NULL		0	NULL	NULL	NULL	gw60_pnas_94_24_12875_s_111	9371768	A gel-mobility shift assay with a radioactive Z-DNA probe and the purified Zalpha nuclease confirms that the Zalpha nuclease binds Z-DNA with a similar affinity to that of the Zalpha domain itself (data not shown).	bind
37617	3	10397	6	NULL	NULL	0	NULL	statement 1	NULL	affinity of	is equal to	NULL				statement 2	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw60_pnas_94_24_12875_s_111	9371768	A gel-mobility shift assay with a radioactive Z-DNA probe and the purified Zalpha nuclease confirms that the Zalpha nuclease binds Z-DNA with a similar affinity to that of the Zalpha domain itself (data not shown).	bind
44126	1	10398	5	11	NULL	NULL	NULL	Hoxc8	GP		bind					OPN	GP			promoter	NULL	in vitro	NULL	NULL	NULL	NULL	gw70_pnas_102_7_2420_s_123	15699330	A gel-shift assay was performed to demonstrate that Hoxc8 binds to the  OPN promoter  in vitro ( ).	bind
37618	1	10398	6	NULL	NULL	0	NULL	Hoxc8	NULL		bind	NULL				OPN	NULL			promoter	NULL	in vitro	0	NULL	NULL	NULL	gw70_pnas_102_7_2420_s_123	15699330	A gel-shift assay was performed to demonstrate that Hoxc8 binds to the  OPN promoter  in vitro ( ).	bind
44168	1	10400	5	11	NULL	NULL	NULL	tetO sequence	GP		bind					tetO	GP				NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_4_8_1328_s_26	16087738	A gene that is placed under the control of a minimal promoter in which all activating sequences have been removed and replaced by the  tetO sequence will be expressed in cells producing tTA, which in the absence of tetracycline binds to  tetO to allow transcription.	bind
44169	2	10400	5	11	NULL	NULL	NULL	statement 3	Process		allows					transcription	Process				NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_4_8_1328_s_26	16087738	A gene that is placed under the control of a minimal promoter in which all activating sequences have been removed and replaced by the  tetO sequence will be expressed in cells producing tTA, which in the absence of tetracycline binds to  tetO to allow transcription.	bind
44170	3	10400	5	11	NULL	NULL	NULL	statement 1	Process		in the absence of					tetracycline	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_4_8_1328_s_26	16087738	A gene that is placed under the control of a minimal promoter in which all activating sequences have been removed and replaced by the  tetO sequence will be expressed in cells producing tTA, which in the absence of tetracycline binds to  tetO to allow transcription.	bind
37941	1	10400	6	NULL	NULL	0	NULL	tetO sequence 	NULL		bind	NULL				tetO	NULL				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_8_1328_s_26	16087738	A gene that is placed under the control of a minimal promoter in which all activating sequences have been removed and replaced by the  tetO sequence will be expressed in cells producing tTA, which in the absence of tetracycline binds to  tetO to allow transcription.	bind
37942	2	10400	6	NULL	NULL	0	NULL	statement 1	NULL		occurs in absence of	NULL				tetracyclin	NULL				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_8_1328_s_26	16087738	A gene that is placed under the control of a minimal promoter in which all activating sequences have been removed and replaced by the  tetO sequence will be expressed in cells producing tTA, which in the absence of tetracycline binds to  tetO to allow transcription.	bind
37943	3	10400	6	NULL	NULL	0	NULL	statement 2	NULL		allows	NULL				transcription	NULL				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_8_1328_s_26	16087738	A gene that is placed under the control of a minimal promoter in which all activating sequences have been removed and replaced by the  tetO sequence will be expressed in cells producing tTA, which in the absence of tetracycline binds to  tetO to allow transcription.	bind
38144	1	10401	6	13	NULL	NULL	NULL	GTP S	Chemical		bind					membrane G proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_40_6_826_s_20	11369036	A general agonist action was investigated by assessing the ability of SKF83959 to stimulate [35]guanosine-5''- O-(3-thio)triphosphate ([35]GTP S) binding to membrane G proteins (  Wang and   Panchalingam).	bind
38145	2	10401	6	13	NULL	NULL	NULL	GTP S	Chemical		is					guanosine-5''- O-(3-thio)triphosphate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_40_6_826_s_20	11369036	A general agonist action was investigated by assessing the ability of SKF83959 to stimulate [35]guanosine-5''- O-(3-thio)triphosphate ([35]GTP S) binding to membrane G proteins (  Wang and   Panchalingam).	bind
44307	1	10401	7	10	NULL	0	NULL	GTP S			bind					membrane G proteins					NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_40_6_826_s_20	11369036	A general agonist action was investigated by assessing the ability of SKF83959 to stimulate [35]guanosine-5''- O-(3-thio)triphosphate ([35]GTP S) binding to membrane G proteins (  Wang and   Panchalingam).	bind
44309	3	10401	7	10	NULL	0	NULL	GTP S			is					guanosine-5''- O-(3-thio)triphosphate					NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_40_6_826_s_20	11369036	A general agonist action was investigated by assessing the ability of SKF83959 to stimulate [35]guanosine-5''- O-(3-thio)triphosphate ([35]GTP S) binding to membrane G proteins (  Wang and   Panchalingam).	bind
38147	1	10402	6	13	NULL	NULL	NULL	PBCV-1 capping enzyme	GP	Chlorella virus	bind		directly			target RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_21_12226_s_26	9770468	A general mechanism for RNA guanylylation, proposed on the basis of the crystal structure of  Chlorella virus PBCV-1 capping enzyme ( 37), suggested direct binding to target RNAs.	bind
44310	1	10402	7	NULL	NULL	0	NULL	 PBCV-1 capping enzyme	NULL	Chlorella virus	bind	NULL	directly			RNA	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_21_12226_s_26	9770468	A general mechanism for RNA guanylylation, proposed on the basis of the crystal structure of  Chlorella virus PBCV-1 capping enzyme ( 37), suggested direct binding to target RNAs.	bind
38384	2	10403	6	13	NULL	NULL	NULL	MeCP2	GP		bind					DNA	NucleicAcid	methylated			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5291_s_20	12954765	A general notion is that MBD proteins bind methylated CpG  in vitro and  in vivo, function in transcriptional repression and are associated with histone deacetylases: when bound to methylated DNA, MeCP2 recruits the SIN3 histone deacetylase- containing complex, while MBD2 and MBD3 interact with the NuRD/Mi2 deacetylase complex ( 11) and MBD1 transcriptional repression has been shown to be deacetylase-dependent ( 12).	bind
38385	3	10403	6	13	NULL	NULL	NULL	MeCP2	GP		recruits					SIN3 histone deacetylase- containing complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5291_s_20	12954765	A general notion is that MBD proteins bind methylated CpG  in vitro and  in vivo, function in transcriptional repression and are associated with histone deacetylases: when bound to methylated DNA, MeCP2 recruits the SIN3 histone deacetylase- containing complex, while MBD2 and MBD3 interact with the NuRD/Mi2 deacetylase complex ( 11) and MBD1 transcriptional repression has been shown to be deacetylase-dependent ( 12).	bind
38386	4	10403	6	13	NULL	NULL	NULL	statement 3	Process		occurs after					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5291_s_20	12954765	A general notion is that MBD proteins bind methylated CpG  in vitro and  in vivo, function in transcriptional repression and are associated with histone deacetylases: when bound to methylated DNA, MeCP2 recruits the SIN3 histone deacetylase- containing complex, while MBD2 and MBD3 interact with the NuRD/Mi2 deacetylase complex ( 11) and MBD1 transcriptional repression has been shown to be deacetylase-dependent ( 12).	bind
38387	5	10403	6	13	NULL	NULL	NULL	MBD2	GP		interacts with					NuRD/Mi2 deacetylase complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5291_s_20	12954765	A general notion is that MBD proteins bind methylated CpG  in vitro and  in vivo, function in transcriptional repression and are associated with histone deacetylases: when bound to methylated DNA, MeCP2 recruits the SIN3 histone deacetylase- containing complex, while MBD2 and MBD3 interact with the NuRD/Mi2 deacetylase complex ( 11) and MBD1 transcriptional repression has been shown to be deacetylase-dependent ( 12).	bind
38389	7	10403	6	13	NULL	NULL	NULL	MBD3	GP		interacts with					NuRD/Mi2 deacetylase complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5291_s_20	12954765	A general notion is that MBD proteins bind methylated CpG  in vitro and  in vivo, function in transcriptional repression and are associated with histone deacetylases: when bound to methylated DNA, MeCP2 recruits the SIN3 histone deacetylase- containing complex, while MBD2 and MBD3 interact with the NuRD/Mi2 deacetylase complex ( 11) and MBD1 transcriptional repression has been shown to be deacetylase-dependent ( 12).	bind
38390	8	10403	6	13	NULL	NULL	NULL	MBD1	GP	transcriptional repression of	is dependent on					deacetylase	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5291_s_20	12954765	A general notion is that MBD proteins bind methylated CpG  in vitro and  in vivo, function in transcriptional repression and are associated with histone deacetylases: when bound to methylated DNA, MeCP2 recruits the SIN3 histone deacetylase- containing complex, while MBD2 and MBD3 interact with the NuRD/Mi2 deacetylase complex ( 11) and MBD1 transcriptional repression has been shown to be deacetylase-dependent ( 12).	bind
50178	1	10403	6	13	NULL	NULL	NULL	MBD proteins	GP		bind							methylated		CpG	NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5291_s_20	12954765	A general notion is that MBD proteins bind methylated CpG  in vitro and  in vivo, function in transcriptional repression and are associated with histone deacetylases: when bound to methylated DNA, MeCP2 recruits the SIN3 histone deacetylase- containing complex, while MBD2 and MBD3 interact with the NuRD/Mi2 deacetylase complex ( 11) and MBD1 transcriptional repression has been shown to be deacetylase-dependent ( 12).	bind
50179	6	10403	6	13	NULL	NULL	NULL	MBD proteins	GP		bind							methylated		CpG	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5291_s_20	12954765	A general notion is that MBD proteins bind methylated CpG  in vitro and  in vivo, function in transcriptional repression and are associated with histone deacetylases: when bound to methylated DNA, MeCP2 recruits the SIN3 histone deacetylase- containing complex, while MBD2 and MBD3 interact with the NuRD/Mi2 deacetylase complex ( 11) and MBD1 transcriptional repression has been shown to be deacetylase-dependent ( 12).	bind
50180	9	10403	6	13	NULL	NULL	NULL	MBD proteins	GP		function in					transcription	Process	repression of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5291_s_20	12954765	A general notion is that MBD proteins bind methylated CpG  in vitro and  in vivo, function in transcriptional repression and are associated with histone deacetylases: when bound to methylated DNA, MeCP2 recruits the SIN3 histone deacetylase- containing complex, while MBD2 and MBD3 interact with the NuRD/Mi2 deacetylase complex ( 11) and MBD1 transcriptional repression has been shown to be deacetylase-dependent ( 12).	bind
50181	10	10403	6	13	NULL	NULL	NULL	MBD proteins	GP		is associated with					histone deacetylases	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5291_s_20	12954765	A general notion is that MBD proteins bind methylated CpG  in vitro and  in vivo, function in transcriptional repression and are associated with histone deacetylases: when bound to methylated DNA, MeCP2 recruits the SIN3 histone deacetylase- containing complex, while MBD2 and MBD3 interact with the NuRD/Mi2 deacetylase complex ( 11) and MBD1 transcriptional repression has been shown to be deacetylase-dependent ( 12).	bind
44311	1	10403	7	NULL	NULL	0	NULL	MBD proteins	NULL		bind	NULL					NULL	methylated		CpG	NULL	in vitro	0	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5291_s_20	12954765	A general notion is that MBD proteins bind methylated CpG  in vitro and  in vivo, function in transcriptional repression and are associated with histone deacetylases: when bound to methylated DNA, MeCP2 recruits the SIN3 histone deacetylase- containing complex, while MBD2 and MBD3 interact with the NuRD/Mi2 deacetylase complex ( 11) and MBD1 transcriptional repression has been shown to be deacetylase-dependent ( 12).	bind
44312	2	10403	7	10	NULL	0	NULL	MBD proteins	NULL		bind	NULL					NULL	methylated		CpG	NULL	in vivo	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5291_s_20	12954765	A general notion is that MBD proteins bind methylated CpG  in vitro and  in vivo, function in transcriptional repression and are associated with histone deacetylases: when bound to methylated DNA, MeCP2 recruits the SIN3 histone deacetylase- containing complex, while MBD2 and MBD3 interact with the NuRD/Mi2 deacetylase complex ( 11) and MBD1 transcriptional repression has been shown to be deacetylase-dependent ( 12).	bind
44313	3	10403	7	NULL	NULL	0	NULL	MBD proteins	NULL		function in	NULL				transcription	NULL	repression of			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5291_s_20	12954765	A general notion is that MBD proteins bind methylated CpG  in vitro and  in vivo, function in transcriptional repression and are associated with histone deacetylases: when bound to methylated DNA, MeCP2 recruits the SIN3 histone deacetylase- containing complex, while MBD2 and MBD3 interact with the NuRD/Mi2 deacetylase complex ( 11) and MBD1 transcriptional repression has been shown to be deacetylase-dependent ( 12).	bind
44314	4	10403	7	10	NULL	0	NULL	MBD proteins	NULL		is associated with	NULL				histone deacetylases	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5291_s_20	12954765	A general notion is that MBD proteins bind methylated CpG  in vitro and  in vivo, function in transcriptional repression and are associated with histone deacetylases: when bound to methylated DNA, MeCP2 recruits the SIN3 histone deacetylase- containing complex, while MBD2 and MBD3 interact with the NuRD/Mi2 deacetylase complex ( 11) and MBD1 transcriptional repression has been shown to be deacetylase-dependent ( 12).	bind
44316	6	10403	7	10	NULL	0	NULL	MBD proteins	NULL		bind	NULL				DNA	NULL	methylated			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5291_s_20	12954765	A general notion is that MBD proteins bind methylated CpG  in vitro and  in vivo, function in transcriptional repression and are associated with histone deacetylases: when bound to methylated DNA, MeCP2 recruits the SIN3 histone deacetylase- containing complex, while MBD2 and MBD3 interact with the NuRD/Mi2 deacetylase complex ( 11) and MBD1 transcriptional repression has been shown to be deacetylase-dependent ( 12).	bind
44317	7	10403	7	NULL	NULL	0	NULL	MeCP2 	NULL		recruits	NULL				SIN3 histone deacetylase- containing complex	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5291_s_20	12954765	A general notion is that MBD proteins bind methylated CpG  in vitro and  in vivo, function in transcriptional repression and are associated with histone deacetylases: when bound to methylated DNA, MeCP2 recruits the SIN3 histone deacetylase- containing complex, while MBD2 and MBD3 interact with the NuRD/Mi2 deacetylase complex ( 11) and MBD1 transcriptional repression has been shown to be deacetylase-dependent ( 12).	bind
44318	8	10403	7	NULL	NULL	0	NULL	statement 7	NULL		occurs upon	NULL				statement 6	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5291_s_20	12954765	A general notion is that MBD proteins bind methylated CpG  in vitro and  in vivo, function in transcriptional repression and are associated with histone deacetylases: when bound to methylated DNA, MeCP2 recruits the SIN3 histone deacetylase- containing complex, while MBD2 and MBD3 interact with the NuRD/Mi2 deacetylase complex ( 11) and MBD1 transcriptional repression has been shown to be deacetylase-dependent ( 12).	bind
44319	9	10403	7	NULL	NULL	0	NULL	MBD2	NULL		interacts with	NULL				NuRD/Mi2 deacetylase complex	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5291_s_20	12954765	A general notion is that MBD proteins bind methylated CpG  in vitro and  in vivo, function in transcriptional repression and are associated with histone deacetylases: when bound to methylated DNA, MeCP2 recruits the SIN3 histone deacetylase- containing complex, while MBD2 and MBD3 interact with the NuRD/Mi2 deacetylase complex ( 11) and MBD1 transcriptional repression has been shown to be deacetylase-dependent ( 12).	bind
44320	10	10403	7	NULL	NULL	0	NULL	MBD3	NULL		interacts with	NULL				NuRD/Mi2 deacetylase complex	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5291_s_20	12954765	A general notion is that MBD proteins bind methylated CpG  in vitro and  in vivo, function in transcriptional repression and are associated with histone deacetylases: when bound to methylated DNA, MeCP2 recruits the SIN3 histone deacetylase- containing complex, while MBD2 and MBD3 interact with the NuRD/Mi2 deacetylase complex ( 11) and MBD1 transcriptional repression has been shown to be deacetylase-dependent ( 12).	bind
44321	11	10403	7	NULL	NULL	0	NULL	MBD1	NULL	transcriptional repression of	depends on	NULL				deacetylase	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_18_5291_s_20	12954765	A general notion is that MBD proteins bind methylated CpG  in vitro and  in vivo, function in transcriptional repression and are associated with histone deacetylases: when bound to methylated DNA, MeCP2 recruits the SIN3 histone deacetylase- containing complex, while MBD2 and MBD3 interact with the NuRD/Mi2 deacetylase complex ( 11) and MBD1 transcriptional repression has been shown to be deacetylase-dependent ( 12).	bind
38148	1	10404	6	13	NULL	NULL	NULL	ZBP-89	GP		bind									GC-rich region	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_32_19955_s_385	9685330	A general scheme has emerged; ZBP-89 binds to a GC-rich region that is within the first 200 base pairs downstream of the transcriptional start site of the gene.	bind
50182	2	10404	6	10	NULL	0	NULL		NULL		is located	NULL			GC-rich region		NULL	downstream of 		transcriptional start site	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_32_19955_s_385	9685330	A general scheme has emerged; ZBP-89 binds to a GC-rich region that is within the first 200 base pairs downstream of the transcriptional start site of the gene.	bind
44322	1	10404	7	10	NULL	0	NULL	ZBP-89	NULL		binds to	NULL					NULL			GC-rich region	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_32_19955_s_385	9685330	A general scheme has emerged; ZBP-89 binds to a GC-rich region that is within the first 200 base pairs downstream of the transcriptional start site of the gene.	bind
50183	1	10404	7	10	NULL	0	NULL		NULL		is located	NULL			GC-rich region		NULL	downstream of		transcriptional start site	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_32_19955_s_385	9685330	A general scheme has emerged; ZBP-89 binds to a GC-rich region that is within the first 200 base pairs downstream of the transcriptional start site of the gene.	bind
38391	1	10405	6	13	NULL	NULL	NULL	IGF	GP		bind					IGF-1R	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_14_3638_s_118	11447105	A general trend established from comparing IGFs binding to IGF-1R, IGF-2R, IR and IGFBPs was that the residues that bind to the type 1 receptor appear to overlap those that bind to the insulin receptor, whereas those that bind to type 2 receptor overlap those that interact with IGF-binding proteins.	bind
38392	2	10405	6	13	NULL	NULL	NULL	IGF	GP		bind					IGF-2R	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_14_3638_s_118	11447105	A general trend established from comparing IGFs binding to IGF-1R, IGF-2R, IR and IGFBPs was that the residues that bind to the type 1 receptor appear to overlap those that bind to the insulin receptor, whereas those that bind to type 2 receptor overlap those that interact with IGF-binding proteins.	bind
38393	3	10405	6	13	NULL	NULL	NULL	IGF	GP		bind					IR	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_14_3638_s_118	11447105	A general trend established from comparing IGFs binding to IGF-1R, IGF-2R, IR and IGFBPs was that the residues that bind to the type 1 receptor appear to overlap those that bind to the insulin receptor, whereas those that bind to type 2 receptor overlap those that interact with IGF-binding proteins.	bind
38394	4	10405	6	13	NULL	NULL	NULL	IGF	GP		bind					IGFBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_14_3638_s_118	11447105	A general trend established from comparing IGFs binding to IGF-1R, IGF-2R, IR and IGFBPs was that the residues that bind to the type 1 receptor appear to overlap those that bind to the insulin receptor, whereas those that bind to type 2 receptor overlap those that interact with IGF-binding proteins.	bind
44323	1	10405	7	NULL	NULL	0	NULL	IGFs	NULL		bind	NULL				IGF-1R	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_20_14_3638_s_118	11447105	A general trend established from comparing IGFs binding to IGF-1R, IGF-2R, IR and IGFBPs was that the residues that bind to the type 1 receptor appear to overlap those that bind to the insulin receptor, whereas those that bind to type 2 receptor overlap those that interact with IGF-binding proteins.	bind
44324	2	10405	7	NULL	NULL	0	NULL	IGFs	NULL		bind	NULL				IGF-2R	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_20_14_3638_s_118	11447105	A general trend established from comparing IGFs binding to IGF-1R, IGF-2R, IR and IGFBPs was that the residues that bind to the type 1 receptor appear to overlap those that bind to the insulin receptor, whereas those that bind to type 2 receptor overlap those that interact with IGF-binding proteins.	bind
44325	3	10405	7	NULL	NULL	0	NULL	IGFs	NULL		bind	NULL				IR	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_20_14_3638_s_118	11447105	A general trend established from comparing IGFs binding to IGF-1R, IGF-2R, IR and IGFBPs was that the residues that bind to the type 1 receptor appear to overlap those that bind to the insulin receptor, whereas those that bind to type 2 receptor overlap those that interact with IGF-binding proteins.	bind
44326	4	10405	7	NULL	NULL	0	NULL	IGFs	NULL		bind	NULL				IGFBPs	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_20_14_3638_s_118	11447105	A general trend established from comparing IGFs binding to IGF-1R, IGF-2R, IR and IGFBPs was that the residues that bind to the type 1 receptor appear to overlap those that bind to the insulin receptor, whereas those that bind to type 2 receptor overlap those that interact with IGF-binding proteins.	bind
48851	5	10405	7	NULL	NULL	0	NULL	type 1 receptor	NULL	binding of	overlap with	NULL		 residues 		insulin receptor	NULL	binding of	residues		NULL		0	NULL	NULL	NULL	gw60_embo_20_14_3638_s_118	11447105	A general trend established from comparing IGFs binding to IGF-1R, IGF-2R, IR and IGFBPs was that the residues that bind to the type 1 receptor appear to overlap those that bind to the insulin receptor, whereas those that bind to type 2 receptor overlap those that interact with IGF-binding proteins.	bind
48852	6	10405	7	NULL	NULL	0	NULL	type 2 receptor	NULL	binding of	overlap with	NULL		residues		IGF-binding proteins	NULL	interaction of	residues		NULL		0	NULL	NULL	NULL	gw60_embo_20_14_3638_s_118	11447105	A general trend established from comparing IGFs binding to IGF-1R, IGF-2R, IR and IGFBPs was that the residues that bind to the type 1 receptor appear to overlap those that bind to the insulin receptor, whereas those that bind to type 2 receptor overlap those that interact with IGF-binding proteins.	bind
38149	1	10406	6	13	NULL	NULL	NULL	TR	GP		bind					TH/bZIP	GP			TRE	NULL	tails of untreated, premetamorphic tadpoles	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_50_41222_s_140	16236718	A generality based on the above data is that the level of TR binding to the TH/bZIP TRE in tails and intestines of untreated, premetamorphic tadpoles was at or marginally above background levels, based on signal from exon 5 and control antibody.	bind
38150	2	10406	6	13	NULL	NULL	NULL	TR	GP		bind					TH/bZIP	GP			TRE	NULL	intestines of untreated, premetamorphic tadpoles	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_50_41222_s_140	16236718	A generality based on the above data is that the level of TR binding to the TH/bZIP TRE in tails and intestines of untreated, premetamorphic tadpoles was at or marginally above background levels, based on signal from exon 5 and control antibody.	bind
44327	1	10406	7	NULL	NULL	0	NULL	TR	NULL		bind	NULL				TH/bZIP	NULL			TRE	NULL	tails of untreated premetamorphic tadpoles	0	NULL	NULL	NULL	gw70_jbiolchem_280_50_41222_s_140	16236718	A generality based on the above data is that the level of TR binding to the TH/bZIP TRE in tails and intestines of untreated, premetamorphic tadpoles was at or marginally above background levels, based on signal from exon 5 and control antibody.	bind
44328	2	10406	7	NULL	NULL	0	NULL	TR	NULL		bind	NULL				TH/bZIP	NULL			TRE	NULL	intestines of untreated premetamorphic tadpoles	0	NULL	NULL	NULL	gw70_jbiolchem_280_50_41222_s_140	16236718	A generality based on the above data is that the level of TR binding to the TH/bZIP TRE in tails and intestines of untreated, premetamorphic tadpoles was at or marginally above background levels, based on signal from exon 5 and control antibody.	bind
38151	1	10407	6	13	NULL	NULL	NULL	clusterin	GP		bind					PEX deposits	OrganismPart				NULL	ocular tissues of PEX eyes	NULL	NULL	NULL	NULL	abs-batch0650-0679_invest-ophthalmol-vis-sci_47_5_16639006_s_9	16639006	A generally  decreased immunoreactivity, but a prominent binding of clusterin to all  PEX deposits, could be observed in ocular tissues of PEX eyes.	bind
44329	1	10407	7	NULL	NULL	0	NULL	clusterin	NULL		bind	NULL				PEX deposits	NULL				NULL	ocular tissues of PEX eyes	0	NULL	NULL	NULL	abs-batch0650-0679_invest-ophthalmol-vis-sci_47_5_16639006_s_9	16639006	A generally  decreased immunoreactivity, but a prominent binding of clusterin to all  PEX deposits, could be observed in ocular tissues of PEX eyes.	bind
38152	1	10408	6	13	NULL	NULL	NULL	Pumilio homolog	GP	Drosophila	bind		specifically			fem-3	GP			PME regulatory element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_2189_s_25	10022905	A genetic screen for recessive mutations that cause failure of the sperm-oocyte switch identified six  mog (for masculinization of the germ line) genes ( 18,  19), while a yeast three-hybrid screen for PME-binding proteins yielded FBF (for  fem-3 binding factor), a homolog of  Drosophila Pumilio that binds specifically to the  fem-3 PME regulatory element ( 46).	bind
50184	2	10408	6	13	NULL	NULL	NULL	PME	GP		bind					FBF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_2189_s_25	10022905	A genetic screen for recessive mutations that cause failure of the sperm-oocyte switch identified six  mog (for masculinization of the germ line) genes ( 18,  19), while a yeast three-hybrid screen for PME-binding proteins yielded FBF (for  fem-3 binding factor), a homolog of  Drosophila Pumilio that binds specifically to the  fem-3 PME regulatory element ( 46).	bind
50185	3	10408	6	13	NULL	NULL	NULL	FBF	GP		is					fem-3 binding factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_2189_s_25	10022905	A genetic screen for recessive mutations that cause failure of the sperm-oocyte switch identified six  mog (for masculinization of the germ line) genes ( 18,  19), while a yeast three-hybrid screen for PME-binding proteins yielded FBF (for  fem-3 binding factor), a homolog of  Drosophila Pumilio that binds specifically to the  fem-3 PME regulatory element ( 46).	bind
44360	1	10408	7	NULL	NULL	0	NULL	PME	NULL		bind	NULL				FBF	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_3_2189_s_25	10022905	A genetic screen for recessive mutations that cause failure of the sperm-oocyte switch identified six  mog (for masculinization of the germ line) genes ( 18,  19), while a yeast three-hybrid screen for PME-binding proteins yielded FBF (for  fem-3 binding factor), a homolog of  Drosophila Pumilio that binds specifically to the  fem-3 PME regulatory element ( 46).	bind
44361	2	10408	7	NULL	NULL	0	NULL	Pumilio homolog 	NULL	Drosophila	bind	NULL	specifically			fem-3	NULL			PME regulatory element	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_3_2189_s_25	10022905	A genetic screen for recessive mutations that cause failure of the sperm-oocyte switch identified six  mog (for masculinization of the germ line) genes ( 18,  19), while a yeast three-hybrid screen for PME-binding proteins yielded FBF (for  fem-3 binding factor), a homolog of  Drosophila Pumilio that binds specifically to the  fem-3 PME regulatory element ( 46).	bind
44362	3	10408	7	NULL	NULL	0	NULL	FBF	NULL		is	NULL				fem-3 binding factor	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_3_2189_s_25	10022905	A genetic screen for recessive mutations that cause failure of the sperm-oocyte switch identified six  mog (for masculinization of the germ line) genes ( 18,  19), while a yeast three-hybrid screen for PME-binding proteins yielded FBF (for  fem-3 binding factor), a homolog of  Drosophila Pumilio that binds specifically to the  fem-3 PME regulatory element ( 46).	bind
38153	1	10409	6	13	NULL	NULL	NULL	COUP-TFII	GP		bind									GIRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_40_28385_s_5	10497199	A genetic screen in yeast has allowed us to identify a novel transcriptional factor binding to the GlRE,  i.e. the chicken ovalbumin upstream promoter-transcription factor II (COUP-TFII).	bind
38154	2	10409	6	13	NULL	NULL	NULL	COUP-TFII	GP		is					chicken ovalbumin upstream promoter-transcription factor II	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_40_28385_s_5	10497199	A genetic screen in yeast has allowed us to identify a novel transcriptional factor binding to the GlRE,  i.e. the chicken ovalbumin upstream promoter-transcription factor II (COUP-TFII).	bind
50186	3	10409	6	13	NULL	NULL	NULL	COUP-TFII \t	GP		is a type of					novel transcriptional factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_40_28385_s_5	10497199	A genetic screen in yeast has allowed us to identify a novel transcriptional factor binding to the GlRE,  i.e. the chicken ovalbumin upstream promoter-transcription factor II (COUP-TFII).	bind
44363	1	10409	7	NULL	NULL	0	NULL	COUP-TFII	NULL		bind	NULL					NULL			GlRE	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_40_28385_s_5	10497199	A genetic screen in yeast has allowed us to identify a novel transcriptional factor binding to the GlRE,  i.e. the chicken ovalbumin upstream promoter-transcription factor II (COUP-TFII).	bind
44364	2	10409	7	10	NULL	0	NULL	COUP-TFII	NULL		is	NULL				chicken ovalbumin upstream promoter-transcription factor II	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_40_28385_s_5	10497199	A genetic screen in yeast has allowed us to identify a novel transcriptional factor binding to the GlRE,  i.e. the chicken ovalbumin upstream promoter-transcription factor II (COUP-TFII).	bind
44365	3	10409	7	NULL	NULL	0	NULL	COUP-TFII	NULL		is a type of	NULL				novel transcriptional factor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_40_28385_s_5	10497199	A genetic screen in yeast has allowed us to identify a novel transcriptional factor binding to the GlRE,  i.e. the chicken ovalbumin upstream promoter-transcription factor II (COUP-TFII).	bind
38155	1	10410	6	13	NULL	NULL	NULL	cellular proteins	GP		bind					RRS	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_pnas_98_26_14991_s_90	11734633	A Genetic Screen to Identify Cellular Proteins That Bind to the RRS  in Vivo.	bind
44366	1	10410	7	NULL	NULL	0	NULL	Cellular Proteins	NULL		bind	NULL				RRS	NULL				NULL	in vivo	0	NULL	NULL	NULL	gw60_pnas_98_26_14991_s_90	11734633	A Genetic Screen to Identify Cellular Proteins That Bind to the RRS  in Vivo.	bind
38395	1	10412	6	13	NULL	NULL	NULL	GFP-beta-CaMKII	GP		does not bind					calmodulin	GP		A303R		NULL		NULL	NULL	NULL	NULL	gw60_science_284_5411_162_s_151	10102820	A GFP-beta-CaMKII deficient in calmodulin binding (A303R) bound effectively to F-actin and failed to dissociate after an increase in Ca2+ concentration ( Fig. 4E,  n = 16).	bind
38396	2	10412	6	13	NULL	NULL	NULL	GFP-beta-CaMKII	GP		bind		effectively			F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5411_162_s_151	10102820	A GFP-beta-CaMKII deficient in calmodulin binding (A303R) bound effectively to F-actin and failed to dissociate after an increase in Ca2+ concentration ( Fig. 4E,  n = 16).	bind
38397	3	10412	6	13	NULL	NULL	NULL	Ca2+	Chemical	increase in;;concentration of	does not dissociate					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5411_162_s_151	10102820	A GFP-beta-CaMKII deficient in calmodulin binding (A303R) bound effectively to F-actin and failed to dissociate after an increase in Ca2+ concentration ( Fig. 4E,  n = 16).	bind
44367	1	10412	7	10	NULL	0	NULL	GFP-beta-CaMKII	NULL		does not bind	NULL				calmodulin	NULL		A303R		NULL		NULL	NULL	NULL	NULL	gw60_science_284_5411_162_s_151	10102820	A GFP-beta-CaMKII deficient in calmodulin binding (A303R) bound effectively to F-actin and failed to dissociate after an increase in Ca2+ concentration ( Fig. 4E,  n = 16).	bind
44368	2	10412	7	NULL	NULL	0	NULL	GFP-beta-CaMKII	NULL		bind	NULL	effectively			F-actin	NULL				NULL		0	NULL	NULL	NULL	gw60_science_284_5411_162_s_151	10102820	A GFP-beta-CaMKII deficient in calmodulin binding (A303R) bound effectively to F-actin and failed to dissociate after an increase in Ca2+ concentration ( Fig. 4E,  n = 16).	bind
44369	3	10412	7	10	NULL	0	NULL	Ca2+	NULL	increase in;;concentration of	does not dissociate	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_science_284_5411_162_s_151	10102820	A GFP-beta-CaMKII deficient in calmodulin binding (A303R) bound effectively to F-actin and failed to dissociate after an increase in Ca2+ concentration ( Fig. 4E,  n = 16).	bind
38156	1	10413	6	13	NULL	NULL	NULL	GHS	GP		bind					GHS-R	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_40441_s_314	11546772	A GHS-R homologue identified in the pufferfish shares 58% identity to human GHS-R and is activated by GHRP-6 and nonpeptidyl GHSs ( 17), suggesting that GHS binding to the GHS-R is not species-specific.	bind
50187	2	10413	6	13	NULL	NULL	NULL	GHS-R homologue	GP	pufferfish	is similar to					GHS-R	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_40441_s_314	11546772	A GHS-R homologue identified in the pufferfish shares 58% identity to human GHS-R and is activated by GHRP-6 and nonpeptidyl GHSs ( 17), suggesting that GHS binding to the GHS-R is not species-specific.	bind
50188	3	10413	6	13	NULL	NULL	NULL	GHRP-6	GP		activates					GHS-R homologue	GP	pufferfish			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_40441_s_314	11546772	A GHS-R homologue identified in the pufferfish shares 58% identity to human GHS-R and is activated by GHRP-6 and nonpeptidyl GHSs ( 17), suggesting that GHS binding to the GHS-R is not species-specific.	bind
50189	4	10413	6	13	NULL	NULL	NULL	nonpeptidyl GHSs	GP		activates					GHS-R homologue	GP	pufferfish			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_40441_s_314	11546772	A GHS-R homologue identified in the pufferfish shares 58% identity to human GHS-R and is activated by GHRP-6 and nonpeptidyl GHSs ( 17), suggesting that GHS binding to the GHS-R is not species-specific.	bind
44370	1	10413	7	NULL	NULL	0	NULL	GHS-R homologue	NULL	pufferfish	is similar to	NULL				GHS-R	NULL	human			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_44_40441_s_314	11546772	A GHS-R homologue identified in the pufferfish shares 58% identity to human GHS-R and is activated by GHRP-6 and nonpeptidyl GHSs ( 17), suggesting that GHS binding to the GHS-R is not species-specific.	bind
44371	2	10413	7	NULL	NULL	0	NULL	GHRP-6	NULL		activates	NULL				GHS-R homologue	NULL	pufferfish			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_44_40441_s_314	11546772	A GHS-R homologue identified in the pufferfish shares 58% identity to human GHS-R and is activated by GHRP-6 and nonpeptidyl GHSs ( 17), suggesting that GHS binding to the GHS-R is not species-specific.	bind
44372	3	10413	7	NULL	NULL	0	NULL	nonpeptidyl GHSs	NULL		activates	NULL				GHS-R homologue	NULL	pufferfish			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_44_40441_s_314	11546772	A GHS-R homologue identified in the pufferfish shares 58% identity to human GHS-R and is activated by GHRP-6 and nonpeptidyl GHSs ( 17), suggesting that GHS binding to the GHS-R is not species-specific.	bind
44373	4	10413	7	NULL	NULL	0	NULL	GHS	NULL		bind	NULL	non species-specific			GHS-R	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_44_40441_s_314	11546772	A GHS-R homologue identified in the pufferfish shares 58% identity to human GHS-R and is activated by GHRP-6 and nonpeptidyl GHSs ( 17), suggesting that GHS binding to the GHS-R is not species-specific.	bind
38398	1	10417	6	13	NULL	NULL	NULL	S2- InsP3R-1	GP		forms fusion protein with			amino acids 1574-1765					glycine-rich motif Gly-Tyr-Gly-Glu-Lys-Gly		NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_281_25_16621795_s_4	16621795	A glutathione  S-transferase fusion protein encompassing amino acids 1574-1765 of the  S2- InsP3R-1 and including the glycine-rich motif Gly-Tyr-Gly-Glu-Lys-Gly  bound ATP specifically as measured by fluorescent trinitrophenyl-ATP binding.	bind
38399	2	10417	6	13	NULL	NULL	NULL	statement 1	GP		bind		specifically			ATP	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_281_25_16621795_s_4	16621795	A glutathione  S-transferase fusion protein encompassing amino acids 1574-1765 of the  S2- InsP3R-1 and including the glycine-rich motif Gly-Tyr-Gly-Glu-Lys-Gly  bound ATP specifically as measured by fluorescent trinitrophenyl-ATP binding.	bind
44375	1	10417	7	NULL	NULL	0	NULL	glutathione S-transferase  protein	NULL		encompass	NULL				S2- InsP3R-1	NULL		amino acids 1574-1765		NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_281_25_16621795_s_4	16621795	A glutathione  S-transferase fusion protein encompassing amino acids 1574-1765 of the  S2- InsP3R-1 and including the glycine-rich motif Gly-Tyr-Gly-Glu-Lys-Gly  bound ATP specifically as measured by fluorescent trinitrophenyl-ATP binding.	bind
44376	2	10417	7	NULL	NULL	0	NULL	glutathione S-transferase  protein	NULL		encompass	NULL					NULL		glycine-rich motif Gly-Tyr-Gly-Glu-Lys-Gly		NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_281_25_16621795_s_4	16621795	A glutathione  S-transferase fusion protein encompassing amino acids 1574-1765 of the  S2- InsP3R-1 and including the glycine-rich motif Gly-Tyr-Gly-Glu-Lys-Gly  bound ATP specifically as measured by fluorescent trinitrophenyl-ATP binding.	bind
44377	3	10417	7	NULL	NULL	0	NULL	statement 1	NULL		occur along with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_281_25_16621795_s_4	16621795	A glutathione  S-transferase fusion protein encompassing amino acids 1574-1765 of the  S2- InsP3R-1 and including the glycine-rich motif Gly-Tyr-Gly-Glu-Lys-Gly  bound ATP specifically as measured by fluorescent trinitrophenyl-ATP binding.	bind
44378	4	10417	7	NULL	NULL	0	NULL	statement 3	NULL		bind	NULL	specifically			ATP	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_281_25_16621795_s_4	16621795	A glutathione  S-transferase fusion protein encompassing amino acids 1574-1765 of the  S2- InsP3R-1 and including the glycine-rich motif Gly-Tyr-Gly-Glu-Lys-Gly  bound ATP specifically as measured by fluorescent trinitrophenyl-ATP binding.	bind
44379	5	10417	7	NULL	NULL	0	NULL	glutathione S-transferase protein	NULL		is a type of	NULL				fusion protein	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_281_25_16621795_s_4	16621795	A glutathione  S-transferase fusion protein encompassing amino acids 1574-1765 of the  S2- InsP3R-1 and including the glycine-rich motif Gly-Tyr-Gly-Glu-Lys-Gly  bound ATP specifically as measured by fluorescent trinitrophenyl-ATP binding.	bind
38157	1	10420	6	13	NULL	NULL	NULL	S2(-) InsP(3)R-1	GP		forms fusion protein with			amino acids 1574-1765					glycine-rich motif Gly-Tyr-Gly-Glu-Lys-Gly		NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_j-biol-chem_281_25_16621795_s_4	16621795	A glutathione S-transferase fusion protein encompassing amino acids 1574-1765  of the S2(-) InsP(3)R-1 and including the glycine-rich motif Gly-Tyr-Gly-Glu-Lys-Gly  bound ATP specifically as measured by fluorescent trinitrophenyl-ATP binding.	bind
38158	2	10420	6	13	NULL	NULL	NULL	statement 1	GP		bind		specifically			ATP	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_j-biol-chem_281_25_16621795_s_4	16621795	A glutathione S-transferase fusion protein encompassing amino acids 1574-1765  of the S2(-) InsP(3)R-1 and including the glycine-rich motif Gly-Tyr-Gly-Glu-Lys-Gly  bound ATP specifically as measured by fluorescent trinitrophenyl-ATP binding.	bind
38400	1	10422	6	13	NULL	NULL	NULL	Glycosulfopeptide	GP		bind			C2-O-sLex at Thr-57		P-selectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39569_s_135	10978329	A Glycosulfopeptide with C2-O-sLex at Thr-57 but Not at Thr-44 Binds to P-selectin--  wo isomeric 35SO3-labeled glycosulfopeptides containing three TyrSO3 residues and a C2-O-sLex at either Thr-57 (3-GSP-6) or Thr-44 (3-GSP-6'') were chromatographed on an affinity column containing sPS at a coupling density of 6.5 mg/ml (Fig.  3).	bind
38401	2	10422	6	13	NULL	NULL	NULL	Glycosulfopeptide	GP		does not bind			C2-O-sLex at Thr-44		P-selectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39569_s_135	10978329	A Glycosulfopeptide with C2-O-sLex at Thr-57 but Not at Thr-44 Binds to P-selectin--  wo isomeric 35SO3-labeled glycosulfopeptides containing three TyrSO3 residues and a C2-O-sLex at either Thr-57 (3-GSP-6) or Thr-44 (3-GSP-6'') were chromatographed on an affinity column containing sPS at a coupling density of 6.5 mg/ml (Fig.  3).	bind
44385	1	10422	7	10	NULL	0	NULL	Glycosulfopeptide	NULL		bind	NULL		C2-O-sLex at Thr-57		P-selectin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39569_s_135	10978329	A Glycosulfopeptide with C2-O-sLex at Thr-57 but Not at Thr-44 Binds to P-selectin--  wo isomeric 35SO3-labeled glycosulfopeptides containing three TyrSO3 residues and a C2-O-sLex at either Thr-57 (3-GSP-6) or Thr-44 (3-GSP-6'') were chromatographed on an affinity column containing sPS at a coupling density of 6.5 mg/ml (Fig.  3).	bind
44386	2	10422	7	10	NULL	0	NULL	Glycosulfopeptide	NULL		does not bind	NULL		C2-O-sLex at Thr-44		P-selectin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_50_39569_s_135	10978329	A Glycosulfopeptide with C2-O-sLex at Thr-57 but Not at Thr-44 Binds to P-selectin--  wo isomeric 35SO3-labeled glycosulfopeptides containing three TyrSO3 residues and a C2-O-sLex at either Thr-57 (3-GSP-6) or Thr-44 (3-GSP-6'') were chromatographed on an affinity column containing sPS at a coupling density of 6.5 mg/ml (Fig.  3).	bind
38159	1	10425	6	13	NULL	NULL	NULL	betaIII spectrin	GP		bind					dynactin	GP		Arp1 subunit 		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_172_5_655_s_154	16505164	A Golgi-associated spectrin isoform, betaIII spectrin, was found to bind to the Arp1 subunit of dynactin ( ,  ), whereas ZW10 binds to the dynamitin subunit ( ).	bind
38160	2	10425	6	13	NULL	NULL	NULL	ZW10	GP		bind					dynactin	GP		dynamitin subunit		NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_172_5_655_s_154	16505164	A Golgi-associated spectrin isoform, betaIII spectrin, was found to bind to the Arp1 subunit of dynactin ( ,  ), whereas ZW10 binds to the dynamitin subunit ( ).	bind
38161	3	10425	6	13	NULL	NULL	NULL	betaIII spectrin	GP		is a type of					Golgi-associated spectrin isoform	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_172_5_655_s_154	16505164	A Golgi-associated spectrin isoform, betaIII spectrin, was found to bind to the Arp1 subunit of dynactin ( ,  ), whereas ZW10 binds to the dynamitin subunit ( ).	bind
44387	1	10425	7	NULL	NULL	0	NULL	betaIII spectrin	NULL		bind	NULL				dynactin	NULL		Arp1 subunit		NULL		0	NULL	NULL	NULL	gw70_cellbiol_172_5_655_s_154	16505164	A Golgi-associated spectrin isoform, betaIII spectrin, was found to bind to the Arp1 subunit of dynactin ( ,  ), whereas ZW10 binds to the dynamitin subunit ( ).	bind
44388	2	10425	7	NULL	NULL	0	NULL	ZW10	NULL		binds to	NULL				dynactin	NULL		dynamitin subunit		NULL		0	NULL	NULL	NULL	gw70_cellbiol_172_5_655_s_154	16505164	A Golgi-associated spectrin isoform, betaIII spectrin, was found to bind to the Arp1 subunit of dynactin ( ,  ), whereas ZW10 binds to the dynamitin subunit ( ).	bind
44389	3	10425	7	NULL	NULL	0	NULL	betaIII spectrin	NULL		is a type of	NULL				Golgi-associated spectrin isoform	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_172_5_655_s_154	16505164	A Golgi-associated spectrin isoform, betaIII spectrin, was found to bind to the Arp1 subunit of dynactin ( ,  ), whereas ZW10 binds to the dynamitin subunit ( ).	bind
38453	1	10426	6	13	NULL	NULL	NULL	titin	GP		bind			N2A domain		Capn3	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_24_9127_s_286	14645524	A good candidate for this Capn3 inhibition is its giant partner, titin, possibly through the N2A domain, which binds Capn3 but is not cleaved by it ( ).	bind
38899	2	10426	6	13	NULL	NULL	NULL	titin	GP		is not cleaved by					Capn3	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_24_9127_s_286	14645524	A good candidate for this Capn3 inhibition is its giant partner, titin, possibly through the N2A domain, which binds Capn3 but is not cleaved by it ( ).	bind
44390	1	10426	7	10	NULL	0	NULL	 Capn3	NULL		binds	NULL				titin	NULL		N2A domain		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_24_9127_s_286	14645524	A good candidate for this Capn3 inhibition is its giant partner, titin, possibly through the N2A domain, which binds Capn3 but is not cleaved by it ( ).	bind
44391	2	10426	7	NULL	NULL	0	NULL	Capn3	NULL		does not cleave	NULL				titin	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_24_9127_s_286	14645524	A good candidate for this Capn3 inhibition is its giant partner, titin, possibly through the N2A domain, which binds Capn3 but is not cleaved by it ( ).	bind
38456	1	10428	6	13	NULL	NULL	NULL	MAP kinase phosphatase	GP		bind					ERK2	GP	mutant	loop L16;; D316N		NULL	yeast	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_45_37885_s_246	16148006	A good correlation was found between the strength of MAP kinase phosphatase binding to ERK2 mutations at the loop L16 (D316N, D319N, D319E, E320A, and E320Q) in yeast and ERK2 cytosolic retention in COS-7 cells (compare  Fig. 4 and  TABLE ONE).	bind
38457	2	10428	6	13	NULL	NULL	NULL	MAP kinase phosphatase	GP		bind					ERK2	GP	mutant	loop L16;; D319N		NULL	yeast	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_45_37885_s_246	16148006	A good correlation was found between the strength of MAP kinase phosphatase binding to ERK2 mutations at the loop L16 (D316N, D319N, D319E, E320A, and E320Q) in yeast and ERK2 cytosolic retention in COS-7 cells (compare  Fig. 4 and  TABLE ONE).	bind
38458	3	10428	6	13	NULL	NULL	NULL	MAP kinase phosphatase	GP		bind					ERK2	GP	mutant	loop L16;; D319E		NULL	Yeast	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_45_37885_s_246	16148006	A good correlation was found between the strength of MAP kinase phosphatase binding to ERK2 mutations at the loop L16 (D316N, D319N, D319E, E320A, and E320Q) in yeast and ERK2 cytosolic retention in COS-7 cells (compare  Fig. 4 and  TABLE ONE).	bind
38459	4	10428	6	13	NULL	NULL	NULL	MAP kinase phosphatase	GP		bind					ERK2	GP	mutant	loop L16;; E320A		NULL	yeast	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_45_37885_s_246	16148006	A good correlation was found between the strength of MAP kinase phosphatase binding to ERK2 mutations at the loop L16 (D316N, D319N, D319E, E320A, and E320Q) in yeast and ERK2 cytosolic retention in COS-7 cells (compare  Fig. 4 and  TABLE ONE).	bind
38461	5	10428	6	13	NULL	NULL	NULL	MAP kinase phosphatase	GP		bind					ERK2	GP	mutant	loop L16;; E320Q		NULL	yeast	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_45_37885_s_246	16148006	A good correlation was found between the strength of MAP kinase phosphatase binding to ERK2 mutations at the loop L16 (D316N, D319N, D319E, E320A, and E320Q) in yeast and ERK2 cytosolic retention in COS-7 cells (compare  Fig. 4 and  TABLE ONE).	bind
44392	1	10428	7	10	NULL	0	NULL	MAP kinase phosphatase			bind					ERK2		mutation of	loop L16;;D316N		NULL	yeast	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_45_37885_s_246	16148006	A good correlation was found between the strength of MAP kinase phosphatase binding to ERK2 mutations at the loop L16 (D316N, D319N, D319E, E320A, and E320Q) in yeast and ERK2 cytosolic retention in COS-7 cells (compare  Fig. 4 and  TABLE ONE).	bind
44393	2	10428	7	10	NULL	0	NULL	MAP kinase phosphatase			bind					ERK2		mutation of	loop L16;;D319N 		NULL	yeast	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_45_37885_s_246	16148006	A good correlation was found between the strength of MAP kinase phosphatase binding to ERK2 mutations at the loop L16 (D316N, D319N, D319E, E320A, and E320Q) in yeast and ERK2 cytosolic retention in COS-7 cells (compare  Fig. 4 and  TABLE ONE).	bind
44394	3	10428	7	10	NULL	0	NULL	MAP kinase phosphatase			bind					ERK2		mutation of	loop L16;;D319E		NULL	yeast	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_45_37885_s_246	16148006	A good correlation was found between the strength of MAP kinase phosphatase binding to ERK2 mutations at the loop L16 (D316N, D319N, D319E, E320A, and E320Q) in yeast and ERK2 cytosolic retention in COS-7 cells (compare  Fig. 4 and  TABLE ONE).	bind
44395	4	10428	7	10	NULL	0	NULL	MAP kinase phosphatase			bind					ERK2		mutation of	loop L16;;E320A		NULL	yeast	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_45_37885_s_246	16148006	A good correlation was found between the strength of MAP kinase phosphatase binding to ERK2 mutations at the loop L16 (D316N, D319N, D319E, E320A, and E320Q) in yeast and ERK2 cytosolic retention in COS-7 cells (compare  Fig. 4 and  TABLE ONE).	bind
44396	5	10428	7	10	NULL	0	NULL	MAP kinase phosphatase			bind					ERK2		mutation of	loop L16;;E320Q		NULL	yeast	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_45_37885_s_246	16148006	A good correlation was found between the strength of MAP kinase phosphatase binding to ERK2 mutations at the loop L16 (D316N, D319N, D319E, E320A, and E320Q) in yeast and ERK2 cytosolic retention in COS-7 cells (compare  Fig. 4 and  TABLE ONE).	bind
38466	1	10429	6	13	NULL	NULL	NULL	hMR	GP	mutant	bind					aldosterone	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_12_3317_s_111	9628869	A good correlation was observed between the decrease in the binding affinity of the mutant hMRs for aldosterone and the decrease in their transactivation capacity.	bind
38467	2	10429	6	13	NULL	NULL	NULL	statement 1	Process	decrease in	corelates with					hMRs	GP	decrease in;;transactivation of			NULL		NULL	NULL	NULL	NULL	gw60_embo_17_12_3317_s_111	9628869	A good correlation was observed between the decrease in the binding affinity of the mutant hMRs for aldosterone and the decrease in their transactivation capacity.	bind
44397	1	10429	7	NULL	NULL	0	NULL	hMRs	NULL	mutant	bind	NULL				aldosterone	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_17_12_3317_s_111	9628869	A good correlation was observed between the decrease in the binding affinity of the mutant hMRs for aldosterone and the decrease in their transactivation capacity.	bind
44398	2	10429	7	10	NULL	0	NULL	statement 1	NULL	decrease in	corelates with	NULL				hMRs	NULL	decrease in;;transactivation of			NULL		NULL	NULL	NULL	NULL	gw60_embo_17_12_3317_s_111	9628869	A good correlation was observed between the decrease in the binding affinity of the mutant hMRs for aldosterone and the decrease in their transactivation capacity.	bind
38163	1	10430	6	13	NULL	NULL	NULL	Ste5	GP		bind					Ste11	GP				NULL	yeast	NULL	NULL	NULL	NULL	gw70_annurevpharmacol_42_0_283_s_438	11807174	A good example derives from the mating  pathway in yeast, where the Ste5 scaffold protein binds the MAPKKK Ste11, the MAPKK  Ste7, and the MAPK Fus3.	bind
38164	2	10430	6	13	NULL	NULL	NULL	Ste5	GP		is a type of					scaffold protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevpharmacol_42_0_283_s_438	11807174	A good example derives from the mating  pathway in yeast, where the Ste5 scaffold protein binds the MAPKKK Ste11, the MAPKK  Ste7, and the MAPK Fus3.	bind
38165	3	10430	6	13	NULL	NULL	NULL	Ste5	GP		bind					Ste7	GP				NULL	yeast	NULL	NULL	NULL	NULL	gw70_annurevpharmacol_42_0_283_s_438	11807174	A good example derives from the mating  pathway in yeast, where the Ste5 scaffold protein binds the MAPKKK Ste11, the MAPKK  Ste7, and the MAPK Fus3.	bind
38166	4	10430	6	13	NULL	NULL	NULL	Ste7	GP		is a type of					MAPKK	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevpharmacol_42_0_283_s_438	11807174	A good example derives from the mating  pathway in yeast, where the Ste5 scaffold protein binds the MAPKKK Ste11, the MAPKK  Ste7, and the MAPK Fus3.	bind
38167	5	10430	6	13	NULL	NULL	NULL	Ste11	GP		is a type of					MAPKKK	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevpharmacol_42_0_283_s_438	11807174	A good example derives from the mating  pathway in yeast, where the Ste5 scaffold protein binds the MAPKKK Ste11, the MAPKK  Ste7, and the MAPK Fus3.	bind
38168	6	10430	6	13	NULL	NULL	NULL	Ste5	GP		bind					Fus3	GP				NULL	yeast	NULL	NULL	NULL	NULL	gw70_annurevpharmacol_42_0_283_s_438	11807174	A good example derives from the mating  pathway in yeast, where the Ste5 scaffold protein binds the MAPKKK Ste11, the MAPKK  Ste7, and the MAPK Fus3.	bind
38169	7	10430	6	13	NULL	NULL	NULL	Fus3	GP		is a type of					MAPK	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevpharmacol_42_0_283_s_438	11807174	A good example derives from the mating  pathway in yeast, where the Ste5 scaffold protein binds the MAPKKK Ste11, the MAPKK  Ste7, and the MAPK Fus3.	bind
44399	1	10430	7	10	NULL	0	NULL	Ste5	NULL		binds	NULL				Ste11	NULL				NULL	yeast	NULL	NULL	NULL	NULL	gw70_annurevpharmacol_42_0_283_s_438	11807174	A good example derives from the mating  pathway in yeast, where the Ste5 scaffold protein binds the MAPKKK Ste11, the MAPKK  Ste7, and the MAPK Fus3.	bind
44400	2	10430	7	10	NULL	0	NULL	Ste5 	NULL		binds	NULL				Ste7	NULL				NULL	yeast	NULL	NULL	NULL	NULL	gw70_annurevpharmacol_42_0_283_s_438	11807174	A good example derives from the mating  pathway in yeast, where the Ste5 scaffold protein binds the MAPKKK Ste11, the MAPKK  Ste7, and the MAPK Fus3.	bind
44401	3	10430	7	10	NULL	0	NULL	Ste5	NULL		binds	NULL				Fus3	NULL				NULL	yeast	NULL	NULL	NULL	NULL	gw70_annurevpharmacol_42_0_283_s_438	11807174	A good example derives from the mating  pathway in yeast, where the Ste5 scaffold protein binds the MAPKKK Ste11, the MAPKK  Ste7, and the MAPK Fus3.	bind
44637	4	10430	7	NULL	NULL	0	NULL	Ste5	NULL		is a type of	NULL				scaffold protein	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevpharmacol_42_0_283_s_438	11807174	A good example derives from the mating  pathway in yeast, where the Ste5 scaffold protein binds the MAPKKK Ste11, the MAPKK  Ste7, and the MAPK Fus3.	bind
50190	5	10430	7	10	NULL	0	NULL	Ste11	NULL		is a type of	NULL				MAPKKK	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevpharmacol_42_0_283_s_438	11807174	A good example derives from the mating  pathway in yeast, where the Ste5 scaffold protein binds the MAPKKK Ste11, the MAPKK  Ste7, and the MAPK Fus3.	bind
50191	6	10430	7	10	NULL	0	NULL	Ste7	NULL		is a type of	NULL				MAPKK	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevpharmacol_42_0_283_s_438	11807174	A good example derives from the mating  pathway in yeast, where the Ste5 scaffold protein binds the MAPKKK Ste11, the MAPKK  Ste7, and the MAPK Fus3.	bind
50192	7	10430	7	10	NULL	0	NULL	Fus3	NULL		is a type of	NULL				MAPK	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevpharmacol_42_0_283_s_438	11807174	A good example derives from the mating  pathway in yeast, where the Ste5 scaffold protein binds the MAPKKK Ste11, the MAPKK  Ste7, and the MAPK Fus3.	bind
38170	1	10431	6	13	NULL	NULL	NULL	Rabenosyn-5	GP		bind					Rab5	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_4_2_153_s_77	12586059	A good example is Rabenosyn-5, which can bind to both Rab5 and Rab4 via distinct binding sites.	bind
38171	2	10431	6	13	NULL	NULL	NULL	Rabenosyn-5	GP		bind					Rab4	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_4_2_153_s_77	12586059	A good example is Rabenosyn-5, which can bind to both Rab5 and Rab4 via distinct binding sites.	bind
38172	3	10431	6	13	NULL	NULL	NULL	statement 1	Process	binding site of	is distinct from					statement 2	Process	binding site of			NULL		NULL	NULL	NULL	NULL	gw60_devcell_4_2_153_s_77	12586059	A good example is Rabenosyn-5, which can bind to both Rab5 and Rab4 via distinct binding sites.	bind
44638	1	10431	7	NULL	NULL	0	NULL	Rabenosyn-5	NULL		bind	NULL				Rab5	NULL				NULL		0	NULL	NULL	NULL	gw60_devcell_4_2_153_s_77	12586059	A good example is Rabenosyn-5, which can bind to both Rab5 and Rab4 via distinct binding sites.	bind
44639	2	10431	7	NULL	NULL	0	NULL	Rabenosyn-5	NULL		bind	NULL				Rab4	NULL				NULL		0	NULL	NULL	NULL	gw60_devcell_4_2_153_s_77	12586059	A good example is Rabenosyn-5, which can bind to both Rab5 and Rab4 via distinct binding sites.	bind
44640	3	10431	7	NULL	NULL	0	NULL	statement 1	NULL	binding site of	is different from	NULL				statement 2	NULL	binding site of			NULL		0	NULL	NULL	NULL	gw60_devcell_4_2_153_s_77	12586059	A good example is Rabenosyn-5, which can bind to both Rab5 and Rab4 via distinct binding sites.	bind
38173	1	10432	6	13	NULL	NULL	NULL	FMOC- l-leucine	Chemical		is a type of					partial PPAR agonist	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_65_0_261_s_178	12518001	A good example of this is given  by the partial PPAR  agonist FMOC- l-leucine, which binds and activates PPAR  with weaker affinity compared with full  agonists ( 78).	bind
38174	2	10432	6	13	NULL	NULL	NULL	FMOC- l-leucine	Chemical		bind					PPAR	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_65_0_261_s_178	12518001	A good example of this is given  by the partial PPAR  agonist FMOC- l-leucine, which binds and activates PPAR  with weaker affinity compared with full  agonists ( 78).	bind
38175	3	10432	6	13	NULL	NULL	NULL	FMOC- l-leucine	Chemical		activates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_65_0_261_s_178	12518001	A good example of this is given  by the partial PPAR  agonist FMOC- l-leucine, which binds and activates PPAR  with weaker affinity compared with full  agonists ( 78).	bind
44641	1	10432	7	10	NULL	0	NULL	FMOC- l-leucine	NULL		bind	NULL				PPAR	NULL				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_65_0_261_s_178	12518001	A good example of this is given  by the partial PPAR  agonist FMOC- l-leucine, which binds and activates PPAR  with weaker affinity compared with full  agonists ( 78).	bind
44642	2	10432	7	NULL	NULL	0	NULL	FMOC- l-leucine	NULL		activates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevphysiol_65_0_261_s_178	12518001	A good example of this is given  by the partial PPAR  agonist FMOC- l-leucine, which binds and activates PPAR  with weaker affinity compared with full  agonists ( 78).	bind
44643	3	10432	7	NULL	NULL	0	NULL	FMOC- l-leucine	NULL		is a type of	NULL				partial PPAR agonist	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevphysiol_65_0_261_s_178	12518001	A good example of this is given  by the partial PPAR  agonist FMOC- l-leucine, which binds and activates PPAR  with weaker affinity compared with full  agonists ( 78).	bind
38193	1	10434	6	13	NULL	NULL	NULL	HSPG	GP	GPI-anchored;;melanoma cells	facilitates					fibronectin	GP	adhesion to 			NULL		NULL	NULL	NULL	NULL	gw60_gene_206_2_255_s_166	9469940	A GPI-anchored HSPG from melanoma cells has been shown to facilitate adhesion to fibronection (  Drake et al., 1992) and bind members of the heparin binding growth factor family (  Brunner et al., 1991).	bind
38195	2	10434	6	13	NULL	NULL	NULL	HSPG	GP	GPI-anchored;;melanoma cells	bind					members of the heparin binding growth factor family	GP				NULL		NULL	NULL	NULL	NULL	gw60_gene_206_2_255_s_166	9469940	A GPI-anchored HSPG from melanoma cells has been shown to facilitate adhesion to fibronection (  Drake et al., 1992) and bind members of the heparin binding growth factor family (  Brunner et al., 1991).	bind
44644	1	10434	7	NULL	NULL	0	NULL	HSPG	NULL	GPI-anchored;; melanoma cells	facilitate	NULL				fibronection	NULL	adhesion to			NULL		NULL	NULL	NULL	NULL	gw60_gene_206_2_255_s_166	9469940	A GPI-anchored HSPG from melanoma cells has been shown to facilitate adhesion to fibronection (  Drake et al., 1992) and bind members of the heparin binding growth factor family (  Brunner et al., 1991).	bind
44645	2	10434	7	NULL	NULL	0	NULL	HSPG	NULL	GPI-anchored;;melanoma cells	bind	NULL				heparin binding growth factor family	NULL				NULL		NULL	NULL	NULL	NULL	gw60_gene_206_2_255_s_166	9469940	A GPI-anchored HSPG from melanoma cells has been shown to facilitate adhesion to fibronection (  Drake et al., 1992) and bind members of the heparin binding growth factor family (  Brunner et al., 1991).	bind
38196	1	10436	6	13	NULL	NULL	NULL	Grb2	GP		bind					proline-rich ligands	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_10_5533_s_146	10318918	A Grb2 mutant containing a point mutation in the N-terminal SH3 domain (W36K), which renders Grb2 unable to bind proline-rich ligands ( 23), exerted significant diminished binding to NS5A (Fig.  3 B Right, lane 4).	bind
38197	2	10436	6	13	NULL	NULL	NULL	Grb2 	GP	mutant	abolishes			N-terminal SH3 domain (W36K)		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_10_5533_s_146	10318918	A Grb2 mutant containing a point mutation in the N-terminal SH3 domain (W36K), which renders Grb2 unable to bind proline-rich ligands ( 23), exerted significant diminished binding to NS5A (Fig.  3 B Right, lane 4).	bind
38198	3	10436	6	13	NULL	NULL	NULL	Grb2	GP		bind								NS5A		NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_10_5533_s_146	10318918	A Grb2 mutant containing a point mutation in the N-terminal SH3 domain (W36K), which renders Grb2 unable to bind proline-rich ligands ( 23), exerted significant diminished binding to NS5A (Fig.  3 B Right, lane 4).	bind
38199	4	10436	6	13	NULL	NULL	NULL	Grb2	GP	mutant	diminishes			N-terminal SH3 domain (W36K)		statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_10_5533_s_146	10318918	A Grb2 mutant containing a point mutation in the N-terminal SH3 domain (W36K), which renders Grb2 unable to bind proline-rich ligands ( 23), exerted significant diminished binding to NS5A (Fig.  3 B Right, lane 4).	bind
44648	1	10436	7	10	NULL	0	NULL	Grb2	NULL	point mutation of	does not bind	NULL		N-terminal SH3 domain (W36K)		proline-rich ligands	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_10_5533_s_146	10318918	A Grb2 mutant containing a point mutation in the N-terminal SH3 domain (W36K), which renders Grb2 unable to bind proline-rich ligands ( 23), exerted significant diminished binding to NS5A (Fig.  3 B Right, lane 4).	bind
44649	2	10436	7	10	NULL	0	NULL	Grb2	NULL	point mutation of	diminishes	NULL		N-terminal SH3 domain (W36K)		NS5A	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_10_5533_s_146	10318918	A Grb2 mutant containing a point mutation in the N-terminal SH3 domain (W36K), which renders Grb2 unable to bind proline-rich ligands ( 23), exerted significant diminished binding to NS5A (Fig.  3 B Right, lane 4).	bind
38471	1	10437	6	13	NULL	NULL	NULL	WGA	GP		is a type of					lectin	GP				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_3_429_s_148	16272577	A great fraction (85-100%) of AChE activity in ANCT, AC, LCC and SCC was bound by LCA and WGA, and no statistically significant differences in the percentage of binding between the above lectins and AChE in the various types of lung samples were observed ( Figure 2).	bind
38472	2	10437	6	13	NULL	NULL	NULL	LCA	GP		is a type of					lectin	GP				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_3_429_s_148	16272577	A great fraction (85-100%) of AChE activity in ANCT, AC, LCC and SCC was bound by LCA and WGA, and no statistically significant differences in the percentage of binding between the above lectins and AChE in the various types of lung samples were observed ( Figure 2).	bind
38474	3	10437	6	13	NULL	NULL	NULL	AChE	GP		bind					LCA	GP				NULL	ANCT	NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_3_429_s_148	16272577	A great fraction (85-100%) of AChE activity in ANCT, AC, LCC and SCC was bound by LCA and WGA, and no statistically significant differences in the percentage of binding between the above lectins and AChE in the various types of lung samples were observed ( Figure 2).	bind
38475	4	10437	6	13	NULL	NULL	NULL	AChE	GP		bind					WGA	GP				NULL	ANCT	NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_3_429_s_148	16272577	A great fraction (85-100%) of AChE activity in ANCT, AC, LCC and SCC was bound by LCA and WGA, and no statistically significant differences in the percentage of binding between the above lectins and AChE in the various types of lung samples were observed ( Figure 2).	bind
38477	5	10437	6	13	NULL	NULL	NULL	AChE	GP		bind					LCA	GP				NULL	AC	NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_3_429_s_148	16272577	A great fraction (85-100%) of AChE activity in ANCT, AC, LCC and SCC was bound by LCA and WGA, and no statistically significant differences in the percentage of binding between the above lectins and AChE in the various types of lung samples were observed ( Figure 2).	bind
38478	6	10437	6	13	NULL	NULL	NULL	AChE	GP		bind					WGA	GP				NULL	AC	NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_3_429_s_148	16272577	A great fraction (85-100%) of AChE activity in ANCT, AC, LCC and SCC was bound by LCA and WGA, and no statistically significant differences in the percentage of binding between the above lectins and AChE in the various types of lung samples were observed ( Figure 2).	bind
38481	7	10437	6	13	NULL	NULL	NULL	AChE	GP		bind					LCA	GP				NULL	LCC	NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_3_429_s_148	16272577	A great fraction (85-100%) of AChE activity in ANCT, AC, LCC and SCC was bound by LCA and WGA, and no statistically significant differences in the percentage of binding between the above lectins and AChE in the various types of lung samples were observed ( Figure 2).	bind
38482	8	10437	6	13	NULL	NULL	NULL	AChE	GP		bind					WGA	GP				NULL	LCC	NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_3_429_s_148	16272577	A great fraction (85-100%) of AChE activity in ANCT, AC, LCC and SCC was bound by LCA and WGA, and no statistically significant differences in the percentage of binding between the above lectins and AChE in the various types of lung samples were observed ( Figure 2).	bind
38483	9	10437	6	13	NULL	NULL	NULL	AChE	GP		bind					LCA	GP				NULL	SCC	NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_3_429_s_148	16272577	A great fraction (85-100%) of AChE activity in ANCT, AC, LCC and SCC was bound by LCA and WGA, and no statistically significant differences in the percentage of binding between the above lectins and AChE in the various types of lung samples were observed ( Figure 2).	bind
38487	10	10437	6	13	NULL	NULL	NULL	AChE	GP		bind					WGA	GP				NULL	SCC	NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_3_429_s_148	16272577	A great fraction (85-100%) of AChE activity in ANCT, AC, LCC and SCC was bound by LCA and WGA, and no statistically significant differences in the percentage of binding between the above lectins and AChE in the various types of lung samples were observed ( Figure 2).	bind
44650	1	10437	7	NULL	NULL	0	NULL	AChE	NULL		bind	NULL				LCA	NULL				NULL	ANCT	NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_3_429_s_148	16272577	A great fraction (85-100%) of AChE activity in ANCT, AC, LCC and SCC was bound by LCA and WGA, and no statistically significant differences in the percentage of binding between the above lectins and AChE in the various types of lung samples were observed ( Figure 2).	bind
44651	2	10437	7	NULL	NULL	0	NULL	AChE	NULL		bind	NULL				LCA	NULL				NULL	AC	NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_3_429_s_148	16272577	A great fraction (85-100%) of AChE activity in ANCT, AC, LCC and SCC was bound by LCA and WGA, and no statistically significant differences in the percentage of binding between the above lectins and AChE in the various types of lung samples were observed ( Figure 2).	bind
44652	3	10437	7	NULL	NULL	0	NULL	AChE	NULL		bind	NULL				LCA	NULL				NULL	LCC	NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_3_429_s_148	16272577	A great fraction (85-100%) of AChE activity in ANCT, AC, LCC and SCC was bound by LCA and WGA, and no statistically significant differences in the percentage of binding between the above lectins and AChE in the various types of lung samples were observed ( Figure 2).	bind
44653	4	10437	7	NULL	NULL	0	NULL	AChE	NULL		bind	NULL				LCA	NULL				NULL	SCC	NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_3_429_s_148	16272577	A great fraction (85-100%) of AChE activity in ANCT, AC, LCC and SCC was bound by LCA and WGA, and no statistically significant differences in the percentage of binding between the above lectins and AChE in the various types of lung samples were observed ( Figure 2).	bind
44654	5	10437	7	NULL	NULL	0	NULL	AChE	NULL		bind	NULL				WGA	NULL				NULL	ANCT	NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_3_429_s_148	16272577	A great fraction (85-100%) of AChE activity in ANCT, AC, LCC and SCC was bound by LCA and WGA, and no statistically significant differences in the percentage of binding between the above lectins and AChE in the various types of lung samples were observed ( Figure 2).	bind
44655	6	10437	7	NULL	NULL	0	NULL	AChE	NULL		bind	NULL				WGA	NULL				NULL	AC	NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_3_429_s_148	16272577	A great fraction (85-100%) of AChE activity in ANCT, AC, LCC and SCC was bound by LCA and WGA, and no statistically significant differences in the percentage of binding between the above lectins and AChE in the various types of lung samples were observed ( Figure 2).	bind
44656	7	10437	7	NULL	NULL	0	NULL	AChE	NULL		bind	NULL				WGA	NULL				NULL	LCC	NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_3_429_s_148	16272577	A great fraction (85-100%) of AChE activity in ANCT, AC, LCC and SCC was bound by LCA and WGA, and no statistically significant differences in the percentage of binding between the above lectins and AChE in the various types of lung samples were observed ( Figure 2).	bind
44657	8	10437	7	NULL	NULL	0	NULL	AChE	NULL		bind	NULL				WGA	NULL				NULL	SCC	NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_3_429_s_148	16272577	A great fraction (85-100%) of AChE activity in ANCT, AC, LCC and SCC was bound by LCA and WGA, and no statistically significant differences in the percentage of binding between the above lectins and AChE in the various types of lung samples were observed ( Figure 2).	bind
50299	9	10437	7	10	NULL	0	NULL	LCA	NULL		is a type of	NULL				lectin	NULL				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_27_3_429_s_148	16272577	A great fraction (85-100%) of AChE activity in ANCT, AC, LCC and SCC was bound by LCA and WGA, and no statistically significant differences in the percentage of binding between the above lectins and AChE in the various types of lung samples were observed ( Figure 2).	bind
50301	10	10437	7	10	NULL	0	NULL	WGA	NULL		is a type of	NULL				lectin	NULL				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_27_3_429_s_148	16272577	A great fraction (85-100%) of AChE activity in ANCT, AC, LCC and SCC was bound by LCA and WGA, and no statistically significant differences in the percentage of binding between the above lectins and AChE in the various types of lung samples were observed ( Figure 2).	bind
38200	1	10438	6	13	NULL	NULL	NULL	curcumin-treated cells	Cell		bind					annexin probe	GP				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_25_11_2155_s_134	15271854	A greater number of curcumin-treated cells than control cells bound the annexin probe, giving them a brilliant green fluorescence at the cell surface.	bind
44658	1	10438	7	10	NULL	0	NULL	curcumin-treated cells	NULL		bind	NULL				annexin probe	NULL				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_25_11_2155_s_134	15271854	A greater number of curcumin-treated cells than control cells bound the annexin probe, giving them a brilliant green fluorescence at the cell surface.	bind
38202	1	10439	6	13	NULL	NULL	NULL	apoE	GP		bind					VLDL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_42_6_959_s_241	11369804	A greater number of peptide molecules compared with apoE (increased ligand-binding domains relative to one apoE) could bind VLDL; thus more Ac-hE18A-NH2-VLDL is taken up than VLDL itself.	bind
38204	2	10439	6	13	NULL	NULL	NULL	peptide molecules	GP		bind					VLDL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_42_6_959_s_241	11369804	A greater number of peptide molecules compared with apoE (increased ligand-binding domains relative to one apoE) could bind VLDL; thus more Ac-hE18A-NH2-VLDL is taken up than VLDL itself.	bind
38205	3	10439	6	13	NULL	NULL	NULL	statement 2	Process		is greater than					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_42_6_959_s_241	11369804	A greater number of peptide molecules compared with apoE (increased ligand-binding domains relative to one apoE) could bind VLDL; thus more Ac-hE18A-NH2-VLDL is taken up than VLDL itself.	bind
38206	4	10439	6	13	NULL	NULL	NULL	statement 2	Process		results in					Ac-hE18A-NH2-VLDL	GP	uptake of 			NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_42_6_959_s_241	11369804	A greater number of peptide molecules compared with apoE (increased ligand-binding domains relative to one apoE) could bind VLDL; thus more Ac-hE18A-NH2-VLDL is taken up than VLDL itself.	bind
38209	5	10439	6	13	NULL	NULL	NULL	statement 2	Process		results in					VLDL	GP	uptake of 			NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_42_6_959_s_241	11369804	A greater number of peptide molecules compared with apoE (increased ligand-binding domains relative to one apoE) could bind VLDL; thus more Ac-hE18A-NH2-VLDL is taken up than VLDL itself.	bind
38210	6	10439	6	13	NULL	NULL	NULL	statement 4	Process		is more than					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_42_6_959_s_241	11369804	A greater number of peptide molecules compared with apoE (increased ligand-binding domains relative to one apoE) could bind VLDL; thus more Ac-hE18A-NH2-VLDL is taken up than VLDL itself.	bind
44659	1	10439	7	NULL	NULL	0	NULL	peptide molecules 	NULL		bind	NULL				VLDL	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_42_6_959_s_241	11369804	A greater number of peptide molecules compared with apoE (increased ligand-binding domains relative to one apoE) could bind VLDL; thus more Ac-hE18A-NH2-VLDL is taken up than VLDL itself.	bind
44660	2	10439	7	NULL	NULL	0	NULL	apoE	NULL		bind	NULL				VLDL	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_42_6_959_s_241	11369804	A greater number of peptide molecules compared with apoE (increased ligand-binding domains relative to one apoE) could bind VLDL; thus more Ac-hE18A-NH2-VLDL is taken up than VLDL itself.	bind
44661	3	10439	7	NULL	NULL	0	NULL	Ac-hE18A-NH2-VLDL	NULL	uptake of	is more than	NULL				VLDL	NULL	uptake of			NULL		0	NULL	NULL	NULL	gw60_jlipidres_42_6_959_s_241	11369804	A greater number of peptide molecules compared with apoE (increased ligand-binding domains relative to one apoE) could bind VLDL; thus more Ac-hE18A-NH2-VLDL is taken up than VLDL itself.	bind
44662	4	10439	7	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_42_6_959_s_241	11369804	A greater number of peptide molecules compared with apoE (increased ligand-binding domains relative to one apoE) could bind VLDL; thus more Ac-hE18A-NH2-VLDL is taken up than VLDL itself.	bind
44663	5	10439	7	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_42_6_959_s_241	11369804	A greater number of peptide molecules compared with apoE (increased ligand-binding domains relative to one apoE) could bind VLDL; thus more Ac-hE18A-NH2-VLDL is taken up than VLDL itself.	bind
38213	1	10440	6	13	NULL	NULL	NULL	postsynaptic gephyrins	GP		bind					GlyR	GP				NULL	transfected neurons	NULL	NULL	NULL	NULL	gw70_jneurosci_24_6_1398_s_6	14960612	A green fluorescent protein (GFP)-tagged gephyrin-binding loop of the GlyR beta subunit (GFP::betaL) was used as a surrogate for full-length receptors to characterize the GlyR binding capacity of postsynaptic gephyrins in transfected neurons.	bind
44666	1	10440	7	10	NULL	0	NULL	GlyR	NULL		bind	NULL				postsynaptic gephyrins	NULL				NULL	transfected neurons	NULL	NULL	NULL	NULL	gw70_jneurosci_24_6_1398_s_6	14960612	A green fluorescent protein (GFP)-tagged gephyrin-binding loop of the GlyR beta subunit (GFP::betaL) was used as a surrogate for full-length receptors to characterize the GlyR binding capacity of postsynaptic gephyrins in transfected neurons.	bind
38214	1	10441	6	13	NULL	NULL	NULL	DsrA	GP		bind		putative;; direct			target mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_18_6179_s_169	15342588	A grey dashed line to the right of DsrA shows putative direct DsrA  binding to other target mRNAs.	bind
44935	1	10441	7	10	NULL	0	NULL	DsrA	NULL		bind	NULL	direct;;putative			target mRNA	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_18_6179_s_169	15342588	A grey dashed line to the right of DsrA shows putative direct DsrA  binding to other target mRNAs.	bind
38216	1	10442	6	13	NULL	NULL	NULL	PHO	GP		bind					GRH	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_4_1434_s_253	16449654	A GRH-PHO complex was clearly observed, along with a concomitant decrease in the unbound probe DNA, indicating that binding of PHO to GRH increases its affinity for DNA (Fig.  6A).	bind
38217	2	10442	6	13	NULL	NULL	NULL	PHO	GP		has affinity for					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_4_1434_s_253	16449654	A GRH-PHO complex was clearly observed, along with a concomitant decrease in the unbound probe DNA, indicating that binding of PHO to GRH increases its affinity for DNA (Fig.  6A).	bind
38218	3	10442	6	13	NULL	NULL	NULL	statement 1	Process		increases					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_4_1434_s_253	16449654	A GRH-PHO complex was clearly observed, along with a concomitant decrease in the unbound probe DNA, indicating that binding of PHO to GRH increases its affinity for DNA (Fig.  6A).	bind
44936	1	10442	7	NULL	NULL	0	NULL	PHO	NULL		bind	NULL				GRH	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_4_1434_s_253	16449654	A GRH-PHO complex was clearly observed, along with a concomitant decrease in the unbound probe DNA, indicating that binding of PHO to GRH increases its affinity for DNA (Fig.  6A).	bind
44937	2	10442	7	NULL	NULL	0	NULL	GRH	NULL		has affinity for	NULL				DNA	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_4_1434_s_253	16449654	A GRH-PHO complex was clearly observed, along with a concomitant decrease in the unbound probe DNA, indicating that binding of PHO to GRH increases its affinity for DNA (Fig.  6A).	bind
44938	3	10442	7	NULL	NULL	0	NULL	statement 1	NULL		increase	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_4_1434_s_253	16449654	A GRH-PHO complex was clearly observed, along with a concomitant decrease in the unbound probe DNA, indicating that binding of PHO to GRH increases its affinity for DNA (Fig.  6A).	bind
38219	1	10445	6	13	NULL	NULL	NULL	Shh	GP	mouse	does not bind		biochemically			Smo	GP	mouse			NULL		NULL	NULL	NULL	NULL	gw60_science_274_5291_1304_s_26	8966601	A group led by Arnon Rosenthal, a molecular neurobiologist at San Francisco's Genentech Inc., reports in  Nature that mouse Shh doesn't bind biochemically to cells producing the mouse version of Smo, but does bind to cells making mouse Ptc.	bind
38220	2	10445	6	13	NULL	NULL	NULL	Shh	GP	mouse	bind		biochemically			Ptc	GP	mouse			NULL		NULL	NULL	NULL	NULL	gw60_science_274_5291_1304_s_26	8966601	A group led by Arnon Rosenthal, a molecular neurobiologist at San Francisco's Genentech Inc., reports in  Nature that mouse Shh doesn't bind biochemically to cells producing the mouse version of Smo, but does bind to cells making mouse Ptc.	bind
44940	1	10445	7	10	NULL	0	NULL	Shh		mouse	does not bind		biochemically			Smo		mouse			NULL		NULL	NULL	NULL	NULL	gw60_science_274_5291_1304_s_26	8966601	A group led by Arnon Rosenthal, a molecular neurobiologist at San Francisco's Genentech Inc., reports in  Nature that mouse Shh doesn't bind biochemically to cells producing the mouse version of Smo, but does bind to cells making mouse Ptc.	bind
44942	2	10445	7	10	NULL	0	NULL	Shh			bind					Ptc		mouse			NULL		NULL	NULL	NULL	NULL	gw60_science_274_5291_1304_s_26	8966601	A group led by Arnon Rosenthal, a molecular neurobiologist at San Francisco's Genentech Inc., reports in  Nature that mouse Shh doesn't bind biochemically to cells producing the mouse version of Smo, but does bind to cells making mouse Ptc.	bind
38221	1	10446	6	13	NULL	NULL	NULL	Yap1p	GP		bind					Xpo1p	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_24_20805_s_31	11303030	A group of conserved cysteine residues adjacent to the NES is required for regulated localization of Yap1p, and oxidation of these cysteines disrupts binding of Yap1p to Xpo1p  in vitro ( 4).	bind
38238	2	10446	6	13	NULL	NULL	NULL				is required for			conserved cysteine residues adjacent to the NES		Yap1p	GP	regulated localization of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_24_20805_s_31	11303030	A group of conserved cysteine residues adjacent to the NES is required for regulated localization of Yap1p, and oxidation of these cysteines disrupts binding of Yap1p to Xpo1p  in vitro ( 4).	bind
38240	3	10446	6	13	NULL	NULL	NULL			oxidation of	disrupts			conserved cysteine residues adjacent to the NES		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_24_20805_s_31	11303030	A group of conserved cysteine residues adjacent to the NES is required for regulated localization of Yap1p, and oxidation of these cysteines disrupts binding of Yap1p to Xpo1p  in vitro ( 4).	bind
44943	1	10446	7	NULL	NULL	0	NULL	Yap1p	NULL		bind	NULL				Xpo1p	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_276_24_20805_s_31	11303030	A group of conserved cysteine residues adjacent to the NES is required for regulated localization of Yap1p, and oxidation of these cysteines disrupts binding of Yap1p to Xpo1p  in vitro ( 4).	bind
44944	2	10446	7	NULL	NULL	0	NULL		NULL	group of	is adjacent to	NULL		conserved cysteine residues			NULL		NES		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_24_20805_s_31	11303030	A group of conserved cysteine residues adjacent to the NES is required for regulated localization of Yap1p, and oxidation of these cysteines disrupts binding of Yap1p to Xpo1p  in vitro ( 4).	bind
44945	3	10446	7	NULL	NULL	0	NULL	statement 2	NULL		is required for	NULL				Yap1p	NULL	regulated localization of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_24_20805_s_31	11303030	A group of conserved cysteine residues adjacent to the NES is required for regulated localization of Yap1p, and oxidation of these cysteines disrupts binding of Yap1p to Xpo1p  in vitro ( 4).	bind
44946	4	10446	7	NULL	NULL	0	NULL	statement 2	NULL	oxidation of	disrupts	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_24_20805_s_31	11303030	A group of conserved cysteine residues adjacent to the NES is required for regulated localization of Yap1p, and oxidation of these cysteines disrupts binding of Yap1p to Xpo1p  in vitro ( 4).	bind
38242	1	10447	6	13	NULL	NULL	NULL	MBD	GP		is					methyl-CpG binding domain protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_40_37936_s_32	12151392	A group of the methyl-CpG binding domain proteins (MBDs) bind preferentially to methylated CpGs ( 27-30), and several of these MBD proteins associate with histone deacetylases or Mi-2, a member of the SWI2/SNF2 family of ATP-dependent chromatin-remodeling proteins ( 31-34).	bind
38243	2	10447	6	13	NULL	NULL	NULL	MBD	GP		bind		preferentially					methylated		CpGs	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_40_37936_s_32	12151392	A group of the methyl-CpG binding domain proteins (MBDs) bind preferentially to methylated CpGs ( 27-30), and several of these MBD proteins associate with histone deacetylases or Mi-2, a member of the SWI2/SNF2 family of ATP-dependent chromatin-remodeling proteins ( 31-34).	bind
38245	3	10447	6	13	NULL	NULL	NULL	MBD proteins	GP		associates with					histone deacetylases	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_40_37936_s_32	12151392	A group of the methyl-CpG binding domain proteins (MBDs) bind preferentially to methylated CpGs ( 27-30), and several of these MBD proteins associate with histone deacetylases or Mi-2, a member of the SWI2/SNF2 family of ATP-dependent chromatin-remodeling proteins ( 31-34).	bind
38246	4	10447	6	13	NULL	NULL	NULL	MBD proteins	GP		associate with					Mi-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_40_37936_s_32	12151392	A group of the methyl-CpG binding domain proteins (MBDs) bind preferentially to methylated CpGs ( 27-30), and several of these MBD proteins associate with histone deacetylases or Mi-2, a member of the SWI2/SNF2 family of ATP-dependent chromatin-remodeling proteins ( 31-34).	bind
38322	5	10447	6	13	NULL	NULL	NULL	Mi-2	GP		is a member of					SWI2/SNF2 family of ATP-dependent chromatin-remodeling protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_40_37936_s_32	12151392	A group of the methyl-CpG binding domain proteins (MBDs) bind preferentially to methylated CpGs ( 27-30), and several of these MBD proteins associate with histone deacetylases or Mi-2, a member of the SWI2/SNF2 family of ATP-dependent chromatin-remodeling proteins ( 31-34).	bind
44947	1	10447	7	10	NULL	0	NULL	MBDs	NULL		bind	NULL	preferentially				NULL	methylated		CpGs	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_40_37936_s_32	12151392	A group of the methyl-CpG binding domain proteins (MBDs) bind preferentially to methylated CpGs ( 27-30), and several of these MBD proteins associate with histone deacetylases or Mi-2, a member of the SWI2/SNF2 family of ATP-dependent chromatin-remodeling proteins ( 31-34).	bind
44948	2	10447	7	NULL	NULL	0	NULL	MBD proteins	NULL		associate with	NULL				histone deacetylases	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_40_37936_s_32	12151392	A group of the methyl-CpG binding domain proteins (MBDs) bind preferentially to methylated CpGs ( 27-30), and several of these MBD proteins associate with histone deacetylases or Mi-2, a member of the SWI2/SNF2 family of ATP-dependent chromatin-remodeling proteins ( 31-34).	bind
44949	4	10447	7	10	NULL	0	NULL	Mi-2	NULL		is a member of	NULL				SWI2/SNF2 family of ATP-dependent chromatin-remodeling proteins	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_40_37936_s_32	12151392	A group of the methyl-CpG binding domain proteins (MBDs) bind preferentially to methylated CpGs ( 27-30), and several of these MBD proteins associate with histone deacetylases or Mi-2, a member of the SWI2/SNF2 family of ATP-dependent chromatin-remodeling proteins ( 31-34).	bind
44951	5	10447	7	NULL	NULL	0	NULL	MBDs	NULL		is	NULL				methyl-CpG binding domain proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_40_37936_s_32	12151392	A group of the methyl-CpG binding domain proteins (MBDs) bind preferentially to methylated CpGs ( 27-30), and several of these MBD proteins associate with histone deacetylases or Mi-2, a member of the SWI2/SNF2 family of ATP-dependent chromatin-remodeling proteins ( 31-34).	bind
44952	6	10447	7	NULL	NULL	0	NULL	MBD proteins	NULL		associate with	NULL				Mi-2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_40_37936_s_32	12151392	A group of the methyl-CpG binding domain proteins (MBDs) bind preferentially to methylated CpGs ( 27-30), and several of these MBD proteins associate with histone deacetylases or Mi-2, a member of the SWI2/SNF2 family of ATP-dependent chromatin-remodeling proteins ( 31-34).	bind
38323	1	10448	6	13	NULL	NULL	NULL	NGF	GP		mediates					survival effect	Process				NULL	neurons	NULL	NULL	NULL	NULL	gw60_neuroscience_107_2_353_s_215	11731109	A growing body of data accumulates concerning the survival effect mediated by NGF in neurons.	bind
44953	1	10448	7	NULL	NULL	0	NULL	NGF	NULL		mediates	NULL				survival effect	NULL				NULL	in neurons	0	NULL	NULL	NULL	gw60_neuroscience_107_2_353_s_215	11731109	A growing body of data accumulates concerning the survival effect mediated by NGF in neurons.	bind
38324	1	10449	6	13	NULL	NULL	NULL	transcription factor	GP		bind									cis-elements	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_259	15718508	A growing body of evidence in all cell types indicates that the binding of transcription factors to  cis-elements and subsequent gene transcription are profoundly affected by the chromatin structure.	bind
38325	2	10449	6	13	NULL	NULL	NULL	statement 1	Process		leads to					gene transcription	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_259	15718508	A growing body of evidence in all cell types indicates that the binding of transcription factors to  cis-elements and subsequent gene transcription are profoundly affected by the chromatin structure.	bind
38326	3	10449	6	13	NULL	NULL	NULL	statement 1	Process		is affected by		profoundly			chromatin structure	Chromosome				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_259	15718508	A growing body of evidence in all cell types indicates that the binding of transcription factors to  cis-elements and subsequent gene transcription are profoundly affected by the chromatin structure.	bind
38327	4	10449	6	13	NULL	NULL	NULL	statement 2	Process		is affected by		profoundly			chromatin structure	Chromosome				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_259	15718508	A growing body of evidence in all cell types indicates that the binding of transcription factors to  cis-elements and subsequent gene transcription are profoundly affected by the chromatin structure.	bind
44954	1	10449	7	10	NULL	0	NULL	 transcription factors 			bind									cis-elements	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_259	15718508	A growing body of evidence in all cell types indicates that the binding of transcription factors to  cis-elements and subsequent gene transcription are profoundly affected by the chromatin structure.	bind
44955	2	10449	7	10	NULL	0	NULL	statement 1	NULL		leads to	NULL				gene transcription	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_259	15718508	A growing body of evidence in all cell types indicates that the binding of transcription factors to  cis-elements and subsequent gene transcription are profoundly affected by the chromatin structure.	bind
44956	3	10449	7	10	NULL	0	NULL	statement 1	NULL		is affected by	NULL	profoundly			chromatin structure	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_259	15718508	A growing body of evidence in all cell types indicates that the binding of transcription factors to  cis-elements and subsequent gene transcription are profoundly affected by the chromatin structure.	bind
50193	4	10449	7	10	NULL	0	NULL	statement 2	NULL		is affected by	NULL	profoundly			chromatin structure	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_96_3_280_s_259	15718508	A growing body of evidence in all cell types indicates that the binding of transcription factors to  cis-elements and subsequent gene transcription are profoundly affected by the chromatin structure.	bind
38328	1	10450	6	13	NULL	NULL	NULL	HSP47	GP		is a type of					collagen binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_16_9637_s_245	9545296	A growing body of evidence is accumulating that suggests a key role for the collagen binding protein HSP47 in the biosynthesis of procollagen ( 36).	bind
38329	2	10450	6	13	NULL	NULL	NULL	HSP47	GP		plays a role in					procollagen	GP	biosynthesis of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_16_9637_s_245	9545296	A growing body of evidence is accumulating that suggests a key role for the collagen binding protein HSP47 in the biosynthesis of procollagen ( 36).	bind
44957	1	10450	7	NULL	NULL	0	NULL	HSP47	NULL		plays a role in	NULL				procollagen	NULL	biosynthesis of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_16_9637_s_245	9545296	A growing body of evidence is accumulating that suggests a key role for the collagen binding protein HSP47 in the biosynthesis of procollagen ( 36).	bind
44958	2	10450	7	NULL	NULL	0	NULL	HSP47	NULL		is a type of	NULL				collagen binding protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_16_9637_s_245	9545296	A growing body of evidence is accumulating that suggests a key role for the collagen binding protein HSP47 in the biosynthesis of procollagen ( 36).	bind
38330	1	10451	6	13	NULL	NULL	NULL	IGFBP4	GP		is					insulin-like growth factor binding protein 4	GP				NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_67_3_1003_s_2	12193414	A growing body of information suggests antigonadotropic and atretogenic roles for granulosa cell-derived insulin-like growth factor binding proteins (IGFBPs) 4 and 5 during ovarian folliculogenesis.	bind
38331	2	10451	6	13	NULL	NULL	NULL	IGFBP5	GP		is					insulin-like growth factor binding protein 5	GP				NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_67_3_1003_s_2	12193414	A growing body of information suggests antigonadotropic and atretogenic roles for granulosa cell-derived insulin-like growth factor binding proteins (IGFBPs) 4 and 5 during ovarian folliculogenesis.	bind
38332	3	10451	6	13	NULL	NULL	NULL	IGFBP-4	GP		is derived from					granulosa cell	Cell				NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_67_3_1003_s_2	12193414	A growing body of information suggests antigonadotropic and atretogenic roles for granulosa cell-derived insulin-like growth factor binding proteins (IGFBPs) 4 and 5 during ovarian folliculogenesis.	bind
38333	4	10451	6	13	NULL	NULL	NULL	IGFBP5	GP		is derived from					granulosa cell	Cell				NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_67_3_1003_s_2	12193414	A growing body of information suggests antigonadotropic and atretogenic roles for granulosa cell-derived insulin-like growth factor binding proteins (IGFBPs) 4 and 5 during ovarian folliculogenesis.	bind
38334	5	10451	6	13	NULL	NULL	NULL	IGFBP4	GP		possess					antigonadotropic role	Process				NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_67_3_1003_s_2	12193414	A growing body of information suggests antigonadotropic and atretogenic roles for granulosa cell-derived insulin-like growth factor binding proteins (IGFBPs) 4 and 5 during ovarian folliculogenesis.	bind
38335	6	10451	6	13	NULL	NULL	NULL	statement 5	Process		occurs during					ovarian folliculogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_67_3_1003_s_2	12193414	A growing body of information suggests antigonadotropic and atretogenic roles for granulosa cell-derived insulin-like growth factor binding proteins (IGFBPs) 4 and 5 during ovarian folliculogenesis.	bind
38336	7	10451	6	13	NULL	NULL	NULL	IGFBP4	GP		possess					atretogenic role	Process				NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_67_3_1003_s_2	12193414	A growing body of information suggests antigonadotropic and atretogenic roles for granulosa cell-derived insulin-like growth factor binding proteins (IGFBPs) 4 and 5 during ovarian folliculogenesis.	bind
38337	8	10451	6	13	NULL	NULL	NULL	statement 7	Process		occurs during					ovarian folliculogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_67_3_1003_s_2	12193414	A growing body of information suggests antigonadotropic and atretogenic roles for granulosa cell-derived insulin-like growth factor binding proteins (IGFBPs) 4 and 5 during ovarian folliculogenesis.	bind
38338	9	10451	6	13	NULL	NULL	NULL	IGFBP5	GP		possess					antigonadotropic role	Process				NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_67_3_1003_s_2	12193414	A growing body of information suggests antigonadotropic and atretogenic roles for granulosa cell-derived insulin-like growth factor binding proteins (IGFBPs) 4 and 5 during ovarian folliculogenesis.	bind
38339	10	10451	6	13	NULL	NULL	NULL	statement 9	Process		occurs during					ovarian folliculogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_67_3_1003_s_2	12193414	A growing body of information suggests antigonadotropic and atretogenic roles for granulosa cell-derived insulin-like growth factor binding proteins (IGFBPs) 4 and 5 during ovarian folliculogenesis.	bind
38340	11	10451	6	13	NULL	NULL	NULL	IGFBP5	GP		possess					atretogenic role	Process				NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_67_3_1003_s_2	12193414	A growing body of information suggests antigonadotropic and atretogenic roles for granulosa cell-derived insulin-like growth factor binding proteins (IGFBPs) 4 and 5 during ovarian folliculogenesis.	bind
38341	12	10451	6	13	NULL	NULL	NULL	statement 11	Process		occurs during					ovarian folliculogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_67_3_1003_s_2	12193414	A growing body of information suggests antigonadotropic and atretogenic roles for granulosa cell-derived insulin-like growth factor binding proteins (IGFBPs) 4 and 5 during ovarian folliculogenesis.	bind
44959	1	10451	7	NULL	NULL	0	NULL	IGFBP4	NULL		is derived from	NULL				granulosa cell	NULL				NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_67_3_1003_s_2	12193414	A growing body of information suggests antigonadotropic and atretogenic roles for granulosa cell-derived insulin-like growth factor binding proteins (IGFBPs) 4 and 5 during ovarian folliculogenesis.	bind
44960	2	10451	7	NULL	NULL	0	NULL	IGFBP5	NULL		is derived from	NULL				granulosa cell	NULL				NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_67_3_1003_s_2	12193414	A growing body of information suggests antigonadotropic and atretogenic roles for granulosa cell-derived insulin-like growth factor binding proteins (IGFBPs) 4 and 5 during ovarian folliculogenesis.	bind
44961	3	10451	7	NULL	NULL	0	NULL	statement 1	NULL		possess	NULL				antigonadotropic role	NULL				NULL		0	NULL	NULL	NULL	gw60_biolreprod_67_3_1003_s_2	12193414	A growing body of information suggests antigonadotropic and atretogenic roles for granulosa cell-derived insulin-like growth factor binding proteins (IGFBPs) 4 and 5 during ovarian folliculogenesis.	bind
44962	4	10451	7	NULL	NULL	0	NULL	statement 1	NULL		possess	NULL				atretogenic role	NULL				NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_67_3_1003_s_2	12193414	A growing body of information suggests antigonadotropic and atretogenic roles for granulosa cell-derived insulin-like growth factor binding proteins (IGFBPs) 4 and 5 during ovarian folliculogenesis.	bind
44963	5	10451	7	NULL	NULL	0	NULL	statement 2	NULL		possess	NULL				antigonadotropic role	NULL				NULL		0	NULL	NULL	NULL	gw60_biolreprod_67_3_1003_s_2	12193414	A growing body of information suggests antigonadotropic and atretogenic roles for granulosa cell-derived insulin-like growth factor binding proteins (IGFBPs) 4 and 5 during ovarian folliculogenesis.	bind
44964	6	10451	7	NULL	NULL	0	NULL	statement 2	NULL		possess	NULL				atretogenic role	NULL				NULL		0	NULL	NULL	NULL	gw60_biolreprod_67_3_1003_s_2	12193414	A growing body of information suggests antigonadotropic and atretogenic roles for granulosa cell-derived insulin-like growth factor binding proteins (IGFBPs) 4 and 5 during ovarian folliculogenesis.	bind
44965	7	10451	7	NULL	NULL	0	NULL	statement 3	NULL		during	NULL				ovarian folliculogenesis	NULL				NULL		0	NULL	NULL	NULL	gw60_biolreprod_67_3_1003_s_2	12193414	A growing body of information suggests antigonadotropic and atretogenic roles for granulosa cell-derived insulin-like growth factor binding proteins (IGFBPs) 4 and 5 during ovarian folliculogenesis.	bind
44966	8	10451	7	NULL	NULL	0	NULL	statement 4	NULL		during	NULL				ovarian folliculogenesis	NULL				NULL		0	NULL	NULL	NULL	gw60_biolreprod_67_3_1003_s_2	12193414	A growing body of information suggests antigonadotropic and atretogenic roles for granulosa cell-derived insulin-like growth factor binding proteins (IGFBPs) 4 and 5 during ovarian folliculogenesis.	bind
44967	9	10451	7	NULL	NULL	0	NULL	statement 5	NULL		during	NULL				ovarian folliculogenesis	NULL				NULL		0	NULL	NULL	NULL	gw60_biolreprod_67_3_1003_s_2	12193414	A growing body of information suggests antigonadotropic and atretogenic roles for granulosa cell-derived insulin-like growth factor binding proteins (IGFBPs) 4 and 5 during ovarian folliculogenesis.	bind
44968	10	10451	7	NULL	NULL	0	NULL	statement 6	NULL		during	NULL				ovarian folliculogenesis	NULL				NULL		0	NULL	NULL	NULL	gw60_biolreprod_67_3_1003_s_2	12193414	A growing body of information suggests antigonadotropic and atretogenic roles for granulosa cell-derived insulin-like growth factor binding proteins (IGFBPs) 4 and 5 during ovarian folliculogenesis.	bind
44969	11	10451	7	NULL	NULL	0	NULL	IGFBP	NULL		is	NULL				insulin-like growth factor binding protein	NULL				NULL		0	NULL	NULL	NULL	gw60_biolreprod_67_3_1003_s_2	12193414	A growing body of information suggests antigonadotropic and atretogenic roles for granulosa cell-derived insulin-like growth factor binding proteins (IGFBPs) 4 and 5 during ovarian folliculogenesis.	bind
38342	1	10452	6	13	NULL	NULL	NULL	human immunodeficiency virus	Organism		bind					DC-SIGN	GP				NULL		NULL	NULL	NULL	NULL	gw70_amjpathol_164_5_1587_s_29	15111305	A growing list of pathogens is bound by DC-SIGN,  including human immunodeficiency virus,  Mycobacterium tuberculosis,   Leishmania amastigotes,   and Dengue virus.	bind
38343	2	10452	6	13	NULL	NULL	NULL	Mycobacterium tuberculosis	Organism		bind					DC-SIGN	GP				NULL		NULL	NULL	NULL	NULL	gw70_amjpathol_164_5_1587_s_29	15111305	A growing list of pathogens is bound by DC-SIGN,  including human immunodeficiency virus,  Mycobacterium tuberculosis,   Leishmania amastigotes,   and Dengue virus.	bind
38344	3	10452	6	13	NULL	NULL	NULL	Leishmania amastigotes	Organism		bind					DC-SIGN	GP				NULL		NULL	NULL	NULL	NULL	gw70_amjpathol_164_5_1587_s_29	15111305	A growing list of pathogens is bound by DC-SIGN,  including human immunodeficiency virus,  Mycobacterium tuberculosis,   Leishmania amastigotes,   and Dengue virus.	bind
38345	4	10452	6	13	NULL	NULL	NULL	Dengue virus	Organism		bind					DC-SIGN	GP				NULL		NULL	NULL	NULL	NULL	gw70_amjpathol_164_5_1587_s_29	15111305	A growing list of pathogens is bound by DC-SIGN,  including human immunodeficiency virus,  Mycobacterium tuberculosis,   Leishmania amastigotes,   and Dengue virus.	bind
44970	1	10452	7	NULL	NULL	0	NULL	DC-SIGN	NULL		bind	NULL				human immunodeficiency virus	NULL				NULL		0	NULL	NULL	NULL	gw70_amjpathol_164_5_1587_s_29	15111305	A growing list of pathogens is bound by DC-SIGN,  including human immunodeficiency virus,  Mycobacterium tuberculosis,   Leishmania amastigotes,   and Dengue virus.	bind
44971	2	10452	7	NULL	NULL	0	NULL	DC-SIGN	NULL		bind	NULL				Mycobacterium tuberculosis	NULL				NULL		0	NULL	NULL	NULL	gw70_amjpathol_164_5_1587_s_29	15111305	A growing list of pathogens is bound by DC-SIGN,  including human immunodeficiency virus,  Mycobacterium tuberculosis,   Leishmania amastigotes,   and Dengue virus.	bind
44972	3	10452	7	NULL	NULL	0	NULL	DC-SIGN	NULL		bind	NULL				Leishmania amastigotes	NULL				NULL		0	NULL	NULL	NULL	gw70_amjpathol_164_5_1587_s_29	15111305	A growing list of pathogens is bound by DC-SIGN,  including human immunodeficiency virus,  Mycobacterium tuberculosis,   Leishmania amastigotes,   and Dengue virus.	bind
44973	4	10452	7	NULL	NULL	0	NULL	DC-SIGN	NULL		bind	NULL				Dengue virus	NULL				NULL		0	NULL	NULL	NULL	gw70_amjpathol_164_5_1587_s_29	15111305	A growing list of pathogens is bound by DC-SIGN,  including human immunodeficiency virus,  Mycobacterium tuberculosis,   Leishmania amastigotes,   and Dengue virus.	bind
38358	1	10454	6	13	NULL	NULL	NULL	GLUT1	GP		is a type of					glucose transporter	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
38359	2	10454	6	13	NULL	NULL	NULL	GLUT1	GP		is a type of					membrane protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
38360	3	10454	6	13	NULL	NULL	NULL	transmembrane Semaphorin-F	GP		is a type of					membrane protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
38361	4	10454	6	13	NULL	NULL	NULL	neurophilin-1	GP		is a type of					membrane protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
38362	5	10454	6	13	NULL	NULL	NULL	syndecan-4	GP		is a type of					membrane protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
38363	6	10454	6	13	NULL	NULL	NULL	tyrosinase-related protein-1	GP		is a type of					membrane protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
38364	7	10454	6	13	NULL	NULL	NULL	alpha5 integrin	GP		is a type of					membrane protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
38365	8	10454	6	13	NULL	NULL	NULL	alpha6 integrin	GP		is a type of					membrane protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
38366	9	10454	6	13	NULL	NULL	NULL	type III transforming growth factor-beta receptor	GP		is a type of					membrane protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
38367	10	10454	6	13	NULL	NULL	NULL	insulin-like growth factor 1 receptor	GP		is a type of					membrane protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
38368	11	10454	6	13	NULL	NULL	NULL	megalin	GP		is a type of					membrane protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
38369	12	10454	6	13	NULL	NULL	NULL	5T4 antigen	GP		is a type of					membrane protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
38370	13	10454	6	13	NULL	NULL	NULL	beta1-adrenergic receptor	GP		is a type of					membrane protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
38371	14	10454	6	13	NULL	NULL	NULL	GIPC	GP		bind			PDZ domain		GLUT1	GP		C-terminus		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
38372	15	10454	6	13	NULL	NULL	NULL	GIPC	GP		bind			PDZ domain		transmembrane Semaphorin-F	GP		C-termini		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
38373	16	10454	6	13	NULL	NULL	NULL	GIPC	GP		bind			PDZ domain		neurophilin-1	GP		C-termini		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
38374	17	10454	6	13	NULL	NULL	NULL	GIPC	GP		bind			PDZ domain		syndecan-4	GP		C-termini		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
38375	18	10454	6	13	NULL	NULL	NULL	GIPC	GP		bind			PDZ domain		tyrosinase-related protein-1	GP		C-termini		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
38376	19	10454	6	13	NULL	NULL	NULL	GIPC	GP		bind			PDZ domain		alpha5 integrin	GP		C-termini		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
38377	20	10454	6	13	NULL	NULL	NULL	GIPC	GP		bind			PDZ domain		alpha6 integrin	GP		C-termini		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
38378	21	10454	6	13	NULL	NULL	NULL	GIPC	GP		bind			PDZ domain		type III transforming growth factor-beta receptor	GP		C-termini		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
38379	22	10454	6	13	NULL	NULL	NULL	GIPC	GP		bind			PDZ domain		insulin-like growth factor 1 receptor	GP		C-termini		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
38380	23	10454	6	13	NULL	NULL	NULL	GIPC	GP		bind			PDZ domain		megalin	GP		C-termini		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
38381	24	10454	6	13	NULL	NULL	NULL	GIPC	GP		bind			PDZ domain		5T4 antigen	GP		C-termini		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
38382	25	10454	6	13	NULL	NULL	NULL	GIPC	GP		bind			PDZ domain		beta1-adrenergic receptor	GP		C-termini		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
44974	1	10454	7	NULL	NULL	0	NULL	GLUT1	NULL		bind	NULL		C terminus		GIPC	NULL		PDZ domain 		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
44975	2	10454	7	NULL	NULL	0	NULL	Semaphorin-F	NULL		bind	NULL		C-terminus		GIPC	NULL		PDZ domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
44994	3	10454	7	NULL	NULL	0	NULL	neurophilin-1	NULL		bind	NULL		C terminus		GIPC	NULL		PDZ domain		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
44997	4	10454	7	NULL	NULL	0	NULL	syndecan-4 	NULL		bind	NULL		C terminus		GIPC	NULL		PDZ domain		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
44998	5	10454	7	NULL	NULL	0	NULL	tyrosinase-related protein-1	NULL		bind	NULL		C terminus		GIPC	NULL		PDZ domain		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
45001	6	10454	7	NULL	NULL	0	NULL	integrin	NULL		bind	NULL		alpha5 subunit		GIPC	NULL		PDZ domain		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
45003	7	10454	7	NULL	NULL	0	NULL	integrin	NULL		bind	NULL		alpha6 subunit		GIPC	NULL		PDZ domain		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
45004	8	10454	7	NULL	NULL	0	NULL	type III transforming growth factor-beta receptor	NULL		bind	NULL		C terminus		GIPC	NULL		PDZ domain		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
45007	9	10454	7	NULL	NULL	0	NULL	insulin-like growth factor 1 receptor 	NULL		bind	NULL		C terminus		GIPC	NULL		PDZ domain		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
45049	10	10454	7	NULL	NULL	0	NULL	megalin	NULL		bind	NULL		C terminus		GIPC	NULL		PDZ domain		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
45050	11	10454	7	NULL	NULL	0	NULL	5T4 antigen	NULL		bind	NULL		C terminus		GIPC	NULL		PDZ domain		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
45051	12	10454	7	NULL	NULL	0	NULL	beta1-adrenergic receptor	NULL		bind	NULL		C terminus		GIPC	NULL		PDZ domain		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
45052	13	10454	7	NULL	NULL	0	NULL	GLUT1	NULL		is a type of	NULL				glucose transporter	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
50286	14	10454	7	NULL	NULL	0	NULL	GLUT1 	NULL		is a type of	NULL				membrane protein	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
50287	15	10454	7	NULL	NULL	0	NULL	Semaphorin-F	NULL		is a type of	NULL				transmembrane protein	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
50288	16	10454	7	NULL	NULL	0	NULL	neurophilin-1	NULL		is a type of	NULL				membrane protein	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
50289	17	10454	7	NULL	NULL	0	NULL	syndecan-4	NULL		is a type of	NULL				membrane protein	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
50290	18	10454	7	NULL	NULL	0	NULL	 tyrosinase-related protein-1	NULL		is a type of	NULL				membrane protein	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
50291	19	10454	7	NULL	NULL	0	NULL	 integrin	NULL		is a type of	NULL				membrane protein	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
50292	20	10454	7	NULL	NULL	0	NULL	type III transforming growth factor-beta receptor	NULL		is a type of	NULL				membrane protein	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
50293	21	10454	7	NULL	NULL	0	NULL	insulin-like growth factor 1 receptor 	NULL		is a type of	NULL				membrane protein	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
50294	22	10454	7	NULL	NULL	0	NULL	megalin	NULL		is a type of	NULL				membrane protein	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
50295	23	10454	7	NULL	NULL	0	NULL	5T4 antigen	NULL		is a type of	NULL				membrane protein	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
50296	24	10454	7	NULL	NULL	0	NULL	beta1-adrenergic receptor	NULL		is a type of	NULL				membrane protein	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_49348_s_269	14507927	A growing number of membrane proteins that bind to the PDZ domain of GIPC through their C termini include the glucose transporter GLUT1 ( ), transmembrane Semaphorin-F ( ), neurophilin-1 ( ), syndecan-4 ( ), tyrosinase-related protein-1 ( ), the alpha5 and alpha6 subunits of integrin ( ), the type III transforming growth factor-beta receptor ( ), the insulin-like growth factor 1 receptor ( ), megalin ( ), the 5T4 antigen ( ), and the beta1-adrenergic receptor ( ).	bind
38348	1	10455	6	13	NULL	NULL	NULL	epidermal growth factor	GP		is a type of					growth factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_24_7_1167_s_181	12807729	A growing number of protein factors are being added to the list of putative  hTERT regulators, including growth factors (e.g. epidermal growth factor) ( ), protein kinases involved in the mitogen-activated protein kinase signaling pathway ( , ) and the stress-activated protein kinase signaling pathway ( ), and an oncogenic, Polycomb group repressor Bmi-1 ( ), which appear to control the  hTERT transcription through the regulation of known or unknown proteins binding to the  hTERT promoter.	bind
38349	2	10455	6	13	NULL	NULL	NULL	Bmi-1	GP		is a type of					polycomb group repressor	GP				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_24_7_1167_s_181	12807729	A growing number of protein factors are being added to the list of putative  hTERT regulators, including growth factors (e.g. epidermal growth factor) ( ), protein kinases involved in the mitogen-activated protein kinase signaling pathway ( , ) and the stress-activated protein kinase signaling pathway ( ), and an oncogenic, Polycomb group repressor Bmi-1 ( ), which appear to control the  hTERT transcription through the regulation of known or unknown proteins binding to the  hTERT promoter.	bind
38350	3	10455	6	13	NULL	NULL	NULL	Bmi-1	GP		control					hTERT	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_24_7_1167_s_181	12807729	A growing number of protein factors are being added to the list of putative  hTERT regulators, including growth factors (e.g. epidermal growth factor) ( ), protein kinases involved in the mitogen-activated protein kinase signaling pathway ( , ) and the stress-activated protein kinase signaling pathway ( ), and an oncogenic, Polycomb group repressor Bmi-1 ( ), which appear to control the  hTERT transcription through the regulation of known or unknown proteins binding to the  hTERT promoter.	bind
38351	4	10455	6	13	NULL	NULL	NULL	protein	GP		bind					hTERT	NucleicAcid			promoter	NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_24_7_1167_s_181	12807729	A growing number of protein factors are being added to the list of putative  hTERT regulators, including growth factors (e.g. epidermal growth factor) ( ), protein kinases involved in the mitogen-activated protein kinase signaling pathway ( , ) and the stress-activated protein kinase signaling pathway ( ), and an oncogenic, Polycomb group repressor Bmi-1 ( ), which appear to control the  hTERT transcription through the regulation of known or unknown proteins binding to the  hTERT promoter.	bind
38352	5	10455	6	13	NULL	NULL	NULL	statement 3	Process		occurs via					statement 4	Process	regulation of			NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_24_7_1167_s_181	12807729	A growing number of protein factors are being added to the list of putative  hTERT regulators, including growth factors (e.g. epidermal growth factor) ( ), protein kinases involved in the mitogen-activated protein kinase signaling pathway ( , ) and the stress-activated protein kinase signaling pathway ( ), and an oncogenic, Polycomb group repressor Bmi-1 ( ), which appear to control the  hTERT transcription through the regulation of known or unknown proteins binding to the  hTERT promoter.	bind
38353	6	10455	6	13	NULL	NULL	NULL	epidermal growth factor	GP		is a type of					putative hTERT regulator	GP				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_24_7_1167_s_181	12807729	A growing number of protein factors are being added to the list of putative  hTERT regulators, including growth factors (e.g. epidermal growth factor) ( ), protein kinases involved in the mitogen-activated protein kinase signaling pathway ( , ) and the stress-activated protein kinase signaling pathway ( ), and an oncogenic, Polycomb group repressor Bmi-1 ( ), which appear to control the  hTERT transcription through the regulation of known or unknown proteins binding to the  hTERT promoter.	bind
38354	7	10455	6	13	NULL	NULL	NULL	Bmi-1	GP		is a type of					putative hTERT regulator	GP				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_24_7_1167_s_181	12807729	A growing number of protein factors are being added to the list of putative  hTERT regulators, including growth factors (e.g. epidermal growth factor) ( ), protein kinases involved in the mitogen-activated protein kinase signaling pathway ( , ) and the stress-activated protein kinase signaling pathway ( ), and an oncogenic, Polycomb group repressor Bmi-1 ( ), which appear to control the  hTERT transcription through the regulation of known or unknown proteins binding to the  hTERT promoter.	bind
38355	8	10455	6	13	NULL	NULL	NULL	stress-activated protein kinase signaling pathway	Process		is a type of					putative hTERT regulator	GP				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_24_7_1167_s_181	12807729	A growing number of protein factors are being added to the list of putative  hTERT regulators, including growth factors (e.g. epidermal growth factor) ( ), protein kinases involved in the mitogen-activated protein kinase signaling pathway ( , ) and the stress-activated protein kinase signaling pathway ( ), and an oncogenic, Polycomb group repressor Bmi-1 ( ), which appear to control the  hTERT transcription through the regulation of known or unknown proteins binding to the  hTERT promoter.	bind
38356	9	10455	6	13	NULL	NULL	NULL	protein kinases	GP		are involved in					mitogen-activated protein kinase signaling pathway	Process				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_24_7_1167_s_181	12807729	A growing number of protein factors are being added to the list of putative  hTERT regulators, including growth factors (e.g. epidermal growth factor) ( ), protein kinases involved in the mitogen-activated protein kinase signaling pathway ( , ) and the stress-activated protein kinase signaling pathway ( ), and an oncogenic, Polycomb group repressor Bmi-1 ( ), which appear to control the  hTERT transcription through the regulation of known or unknown proteins binding to the  hTERT promoter.	bind
38357	10	10455	6	13	NULL	NULL	NULL	statement 9	GP		is a type of					putative hTERT regulator	GP				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_24_7_1167_s_181	12807729	A growing number of protein factors are being added to the list of putative  hTERT regulators, including growth factors (e.g. epidermal growth factor) ( ), protein kinases involved in the mitogen-activated protein kinase signaling pathway ( , ) and the stress-activated protein kinase signaling pathway ( ), and an oncogenic, Polycomb group repressor Bmi-1 ( ), which appear to control the  hTERT transcription through the regulation of known or unknown proteins binding to the  hTERT promoter.	bind
45055	1	10455	7	NULL	NULL	0	NULL	epidermal growth factor	NULL		is a type of	NULL				growth factor	NULL				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_24_7_1167_s_181	12807729	A growing number of protein factors are being added to the list of putative  hTERT regulators, including growth factors (e.g. epidermal growth factor) ( ), protein kinases involved in the mitogen-activated protein kinase signaling pathway ( , ) and the stress-activated protein kinase signaling pathway ( ), and an oncogenic, Polycomb group repressor Bmi-1 ( ), which appear to control the  hTERT transcription through the regulation of known or unknown proteins binding to the  hTERT promoter.	bind
45056	2	10455	7	NULL	NULL	0	NULL	epidermal growth factor	NULL		is a type of	NULL				putative hTERT regulator	NULL				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_24_7_1167_s_181	12807729	A growing number of protein factors are being added to the list of putative  hTERT regulators, including growth factors (e.g. epidermal growth factor) ( ), protein kinases involved in the mitogen-activated protein kinase signaling pathway ( , ) and the stress-activated protein kinase signaling pathway ( ), and an oncogenic, Polycomb group repressor Bmi-1 ( ), which appear to control the  hTERT transcription through the regulation of known or unknown proteins binding to the  hTERT promoter.	bind
45058	3	10455	7	NULL	NULL	0	NULL	protein kinases	NULL		involved in	NULL				mitogen-activated protein kinase signaling pathway	NULL				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_24_7_1167_s_181	12807729	A growing number of protein factors are being added to the list of putative  hTERT regulators, including growth factors (e.g. epidermal growth factor) ( ), protein kinases involved in the mitogen-activated protein kinase signaling pathway ( , ) and the stress-activated protein kinase signaling pathway ( ), and an oncogenic, Polycomb group repressor Bmi-1 ( ), which appear to control the  hTERT transcription through the regulation of known or unknown proteins binding to the  hTERT promoter.	bind
45059	4	10455	7	NULL	NULL	0	NULL	statement 3	NULL		is a type of	NULL				putative hTERT regulator	NULL				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_24_7_1167_s_181	12807729	A growing number of protein factors are being added to the list of putative  hTERT regulators, including growth factors (e.g. epidermal growth factor) ( ), protein kinases involved in the mitogen-activated protein kinase signaling pathway ( , ) and the stress-activated protein kinase signaling pathway ( ), and an oncogenic, Polycomb group repressor Bmi-1 ( ), which appear to control the  hTERT transcription through the regulation of known or unknown proteins binding to the  hTERT promoter.	bind
45062	5	10455	7	NULL	NULL	0	NULL	protein kinases	NULL		involved in	NULL				stress-activated protein kinase signaling pathway	NULL				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_24_7_1167_s_181	12807729	A growing number of protein factors are being added to the list of putative  hTERT regulators, including growth factors (e.g. epidermal growth factor) ( ), protein kinases involved in the mitogen-activated protein kinase signaling pathway ( , ) and the stress-activated protein kinase signaling pathway ( ), and an oncogenic, Polycomb group repressor Bmi-1 ( ), which appear to control the  hTERT transcription through the regulation of known or unknown proteins binding to the  hTERT promoter.	bind
45064	6	10455	7	NULL	NULL	0	NULL	statement 5	NULL		is a type of	NULL				putative hTERT regulator	NULL				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_24_7_1167_s_181	12807729	A growing number of protein factors are being added to the list of putative  hTERT regulators, including growth factors (e.g. epidermal growth factor) ( ), protein kinases involved in the mitogen-activated protein kinase signaling pathway ( , ) and the stress-activated protein kinase signaling pathway ( ), and an oncogenic, Polycomb group repressor Bmi-1 ( ), which appear to control the  hTERT transcription through the regulation of known or unknown proteins binding to the  hTERT promoter.	bind
45066	7	10455	7	NULL	NULL	0	NULL	Bmi-1	NULL		is a type of	NULL				oncogenic Polycomb group repressor 	NULL				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_24_7_1167_s_181	12807729	A growing number of protein factors are being added to the list of putative  hTERT regulators, including growth factors (e.g. epidermal growth factor) ( ), protein kinases involved in the mitogen-activated protein kinase signaling pathway ( , ) and the stress-activated protein kinase signaling pathway ( ), and an oncogenic, Polycomb group repressor Bmi-1 ( ), which appear to control the  hTERT transcription through the regulation of known or unknown proteins binding to the  hTERT promoter.	bind
45067	8	10455	7	NULL	NULL	0	NULL	Bmi-1	NULL		control	NULL				hTERT	NULL	transcription of			NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_24_7_1167_s_181	12807729	A growing number of protein factors are being added to the list of putative  hTERT regulators, including growth factors (e.g. epidermal growth factor) ( ), protein kinases involved in the mitogen-activated protein kinase signaling pathway ( , ) and the stress-activated protein kinase signaling pathway ( ), and an oncogenic, Polycomb group repressor Bmi-1 ( ), which appear to control the  hTERT transcription through the regulation of known or unknown proteins binding to the  hTERT promoter.	bind
45068	9	10455	7	NULL	NULL	0	NULL	proteins	NULL		bind	NULL				hTERT	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_24_7_1167_s_181	12807729	A growing number of protein factors are being added to the list of putative  hTERT regulators, including growth factors (e.g. epidermal growth factor) ( ), protein kinases involved in the mitogen-activated protein kinase signaling pathway ( , ) and the stress-activated protein kinase signaling pathway ( ), and an oncogenic, Polycomb group repressor Bmi-1 ( ), which appear to control the  hTERT transcription through the regulation of known or unknown proteins binding to the  hTERT promoter.	bind
45069	10	10455	7	NULL	NULL	0	NULL	statement 8	NULL		occur through	NULL				statement 9	NULL				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_24_7_1167_s_181	12807729	A growing number of protein factors are being added to the list of putative  hTERT regulators, including growth factors (e.g. epidermal growth factor) ( ), protein kinases involved in the mitogen-activated protein kinase signaling pathway ( , ) and the stress-activated protein kinase signaling pathway ( ), and an oncogenic, Polycomb group repressor Bmi-1 ( ), which appear to control the  hTERT transcription through the regulation of known or unknown proteins binding to the  hTERT promoter.	bind
38346	1	10457	6	13	NULL	NULL	NULL	growth factor receptor-bound protein 2	GP		bind			SH3 domain		SOS	GP				NULL		NULL	NULL	NULL	NULL	gw70_jimmunol_177_1_147_s_166	16785509	A growth factor receptor-bound protein 2 binds to a guanine nucleotide-exchange factor SOS through the SH3 domain.	bind
38347	2	10457	6	13	NULL	NULL	NULL	SOS	GP		is a type of					guanine nucleotide-exchange factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_jimmunol_177_1_147_s_166	16785509	A growth factor receptor-bound protein 2 binds to a guanine nucleotide-exchange factor SOS through the SH3 domain.	bind
45071	1	10457	7	NULL	NULL	0	NULL	growth factor receptor-bound protein 2	NULL		bind	NULL		SH3 domain		SOS	NULL				NULL		0	NULL	NULL	NULL	gw70_jimmunol_177_1_147_s_166	16785509	A growth factor receptor-bound protein 2 binds to a guanine nucleotide-exchange factor SOS through the SH3 domain.	bind
45072	2	10457	7	NULL	NULL	0	NULL	SOS	NULL		is a type of	NULL				guanine nucleotide-exchange factor	NULL				NULL		0	NULL	NULL	NULL	gw70_jimmunol_177_1_147_s_166	16785509	A growth factor receptor-bound protein 2 binds to a guanine nucleotide-exchange factor SOS through the SH3 domain.	bind
39060	1	10458	6	13	NULL	NULL	NULL	NR2B	GP		is expressed in					COS7 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_19_11_4189_s_239	10341223	A GST fusion containing only the PDZ domain of MALS-2 [GST:MALS-2(PDZ)] binds NR2B expressed in COS7 cells, whereas an MALS-2 construct containing only the unique N-terminal region [GST:MALS-2(N70)] is inactive (Fig.  9 A).	bind
39061	2	10458	6	13	NULL	NULL	NULL	GST-fusion protein	GP		contains					MALS-2	GP		PDZ domain		NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_19_11_4189_s_239	10341223	A GST fusion containing only the PDZ domain of MALS-2 [GST:MALS-2(PDZ)] binds NR2B expressed in COS7 cells, whereas an MALS-2 construct containing only the unique N-terminal region [GST:MALS-2(N70)] is inactive (Fig.  9 A).	bind
39062	3	10458	6	13	NULL	NULL	NULL	statement 2	GP		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_19_11_4189_s_239	10341223	A GST fusion containing only the PDZ domain of MALS-2 [GST:MALS-2(PDZ)] binds NR2B expressed in COS7 cells, whereas an MALS-2 construct containing only the unique N-terminal region [GST:MALS-2(N70)] is inactive (Fig.  9 A).	bind
39063	4	10458	6	13	NULL	NULL	NULL	GST:MALS-2(PDZ)	GP		is					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_19_11_4189_s_239	10341223	A GST fusion containing only the PDZ domain of MALS-2 [GST:MALS-2(PDZ)] binds NR2B expressed in COS7 cells, whereas an MALS-2 construct containing only the unique N-terminal region [GST:MALS-2(N70)] is inactive (Fig.  9 A).	bind
39064	5	10458	6	13	NULL	NULL	NULL	MALS-2 construct	GP		contains							unique	N-terminal region		NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_19_11_4189_s_239	10341223	A GST fusion containing only the PDZ domain of MALS-2 [GST:MALS-2(PDZ)] binds NR2B expressed in COS7 cells, whereas an MALS-2 construct containing only the unique N-terminal region [GST:MALS-2(N70)] is inactive (Fig.  9 A).	bind
39065	6	10458	6	13	NULL	NULL	NULL	GST:MALS-2(N70)	GP		is					statement 5	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_19_11_4189_s_239	10341223	A GST fusion containing only the PDZ domain of MALS-2 [GST:MALS-2(PDZ)] binds NR2B expressed in COS7 cells, whereas an MALS-2 construct containing only the unique N-terminal region [GST:MALS-2(N70)] is inactive (Fig.  9 A).	bind
39066	7	10458	6	13	NULL	NULL	NULL	statement 5	GP		is					inactive					NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_19_11_4189_s_239	10341223	A GST fusion containing only the PDZ domain of MALS-2 [GST:MALS-2(PDZ)] binds NR2B expressed in COS7 cells, whereas an MALS-2 construct containing only the unique N-terminal region [GST:MALS-2(N70)] is inactive (Fig.  9 A).	bind
45073	1	10458	7	NULL	NULL	0	NULL	NR2B	NULL		is expressed in	NULL				COS7 cells	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_11_4189_s_239	10341223	A GST fusion containing only the PDZ domain of MALS-2 [GST:MALS-2(PDZ)] binds NR2B expressed in COS7 cells, whereas an MALS-2 construct containing only the unique N-terminal region [GST:MALS-2(N70)] is inactive (Fig.  9 A).	bind
45074	2	10458	7	NULL	NULL	0	NULL	GST:MALS-2(PDZ)	NULL		bind	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_11_4189_s_239	10341223	A GST fusion containing only the PDZ domain of MALS-2 [GST:MALS-2(PDZ)] binds NR2B expressed in COS7 cells, whereas an MALS-2 construct containing only the unique N-terminal region [GST:MALS-2(N70)] is inactive (Fig.  9 A).	bind
45076	3	10458	7	NULL	NULL	0	NULL	GST:MALS-2(N70)	NULL		contains	NULL				MALS-2 construct	NULL		unique N-terminal region 		NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_11_4189_s_239	10341223	A GST fusion containing only the PDZ domain of MALS-2 [GST:MALS-2(PDZ)] binds NR2B expressed in COS7 cells, whereas an MALS-2 construct containing only the unique N-terminal region [GST:MALS-2(N70)] is inactive (Fig.  9 A).	bind
45077	4	10458	7	NULL	NULL	0	NULL	statement 3	NULL		is a type of	NULL				inactive construct	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_11_4189_s_239	10341223	A GST fusion containing only the PDZ domain of MALS-2 [GST:MALS-2(PDZ)] binds NR2B expressed in COS7 cells, whereas an MALS-2 construct containing only the unique N-terminal region [GST:MALS-2(N70)] is inactive (Fig.  9 A).	bind
45078	5	10458	7	NULL	NULL	0	NULL	GST:MALS-2(PDZ)	NULL		contains	NULL				MALS-2	NULL		PDZ domain		NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_11_4189_s_239	10341223	A GST fusion containing only the PDZ domain of MALS-2 [GST:MALS-2(PDZ)] binds NR2B expressed in COS7 cells, whereas an MALS-2 construct containing only the unique N-terminal region [GST:MALS-2(N70)] is inactive (Fig.  9 A).	bind
38498	1	10459	6	13	NULL	NULL	NULL	deltakinase MEK5	GP		bind					ERK5	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_6_2065_s_55	16507987	A GST fusion of MEK5 residues 18 to 165 (deltakinase MEK5) that includes the PB1 domain, but not the kinase domain binds ERK5 (Fig.  1A).	bind
39067	2	10459	6	13	NULL	NULL	NULL	deltakinase MEK5	GP		is a type of					GST fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_6_2065_s_55	16507987	A GST fusion of MEK5 residues 18 to 165 (deltakinase MEK5) that includes the PB1 domain, but not the kinase domain binds ERK5 (Fig.  1A).	bind
39068	3	10459	6	13	NULL	NULL	NULL	deltakinase MEK5	GP		includes								PB1 domain		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_6_2065_s_55	16507987	A GST fusion of MEK5 residues 18 to 165 (deltakinase MEK5) that includes the PB1 domain, but not the kinase domain binds ERK5 (Fig.  1A).	bind
39069	4	10459	6	13	NULL	NULL	NULL	deltakinase MEK5	GP		does not include								kinase domain		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_6_2065_s_55	16507987	A GST fusion of MEK5 residues 18 to 165 (deltakinase MEK5) that includes the PB1 domain, but not the kinase domain binds ERK5 (Fig.  1A).	bind
50194	1	10459	6	13	NULL	NULL	NULL	deltakinase MEK5	GP		contains					MEK5	GP		18-165		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_6_2065_s_55	16507987	A GST fusion of MEK5 residues 18 to 165 (deltakinase MEK5) that includes the PB1 domain, but not the kinase domain binds ERK5 (Fig.  1A).	bind
45079	1	10459	7	NULL	NULL	0	NULL	deltakinase MEK5	NULL		contains	NULL				MEK5 residues	NULL		18-165		NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_6_2065_s_55	16507987	A GST fusion of MEK5 residues 18 to 165 (deltakinase MEK5) that includes the PB1 domain, but not the kinase domain binds ERK5 (Fig.  1A).	bind
45080	2	10459	7	NULL	NULL	0	NULL	deltakinase MEK5	NULL		contains	NULL					NULL		PB1 domain		NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_6_2065_s_55	16507987	A GST fusion of MEK5 residues 18 to 165 (deltakinase MEK5) that includes the PB1 domain, but not the kinase domain binds ERK5 (Fig.  1A).	bind
45082	3	10459	7	10	NULL	0	NULL	deltakinase MEK5	NULL		does not contain	NULL					NULL		kinase domain		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_6_2065_s_55	16507987	A GST fusion of MEK5 residues 18 to 165 (deltakinase MEK5) that includes the PB1 domain, but not the kinase domain binds ERK5 (Fig.  1A).	bind
45084	4	10459	7	10	NULL	0	NULL	deltakinase MEK5	NULL		binds	NULL				ERK5	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_6_2065_s_55	16507987	A GST fusion of MEK5 residues 18 to 165 (deltakinase MEK5) that includes the PB1 domain, but not the kinase domain binds ERK5 (Fig.  1A).	bind
45085	5	10459	7	10	NULL	0	NULL	deltakinase MEK5	NULL		is a type of	NULL				GST fusion protein	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_6_2065_s_55	16507987	A GST fusion of MEK5 residues 18 to 165 (deltakinase MEK5) that includes the PB1 domain, but not the kinase domain binds ERK5 (Fig.  1A).	bind
38512	2	10460	6	13	NULL	NULL	NULL	statement 1	GP		bind					Axin-RGS	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_10_2270_s_71	10811618	A GST fusion of the 25 amino acid APC SAMP3 repeat alone bound to Axin-RGS as well as the longest fragment tested (Figure  2B).	bind
50195	1	10460	6	13	NULL	NULL	NULL	GST fusion protein	GP		contains					APC	GP		SAMP3 repeat 		NULL		NULL	NULL	NULL	NULL	gw60_embo_19_10_2270_s_71	10811618	A GST fusion of the 25 amino acid APC SAMP3 repeat alone bound to Axin-RGS as well as the longest fragment tested (Figure  2B).	bind
45086	1	10460	7	10	NULL	0	NULL	GST fusion protein			contains					APC			SAMP3 repeat		NULL		NULL	NULL	NULL	NULL	gw60_embo_19_10_2270_s_71	10811618	A GST fusion of the 25 amino acid APC SAMP3 repeat alone bound to Axin-RGS as well as the longest fragment tested (Figure  2B).	bind
45087	2	10460	7	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL				Axin-RGS	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_19_10_2270_s_71	10811618	A GST fusion of the 25 amino acid APC SAMP3 repeat alone bound to Axin-RGS as well as the longest fragment tested (Figure  2B).	bind
39070	1	10461	6	13	NULL	NULL	NULL	amphiphysin 1	GP		bind			first 150 amino acids		amphiphysin 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5378_821_s_65	9694653	A GST fusion protein comprising the first 150 amino acids of amphiphysin 1 bound to both amphiphysins 1 and 2 in an overlay assay ( Fig. 2B), indicating that dimerization is mediated by this coiled-coil region of amphiphysin; this suggests the possibility that both heterodimers and homodimers are present.	bind
39071	2	10461	6	13	NULL	NULL	NULL	statement 1	Process		is					homodimerization	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5378_821_s_65	9694653	A GST fusion protein comprising the first 150 amino acids of amphiphysin 1 bound to both amphiphysins 1 and 2 in an overlay assay ( Fig. 2B), indicating that dimerization is mediated by this coiled-coil region of amphiphysin; this suggests the possibility that both heterodimers and homodimers are present.	bind
39072	3	10461	6	13	NULL	NULL	NULL	amphiphysin 1	GP		bind			first 150 amino acids		amphiphysin 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5378_821_s_65	9694653	A GST fusion protein comprising the first 150 amino acids of amphiphysin 1 bound to both amphiphysins 1 and 2 in an overlay assay ( Fig. 2B), indicating that dimerization is mediated by this coiled-coil region of amphiphysin; this suggests the possibility that both heterodimers and homodimers are present.	bind
39073	4	10461	6	13	NULL	NULL	NULL	amphiphysin	GP		mediates			coiled-coil region		amphiphysin	GP	dimerization of			NULL		NULL	NULL	NULL	NULL	gw60_science_281_5378_821_s_65	9694653	A GST fusion protein comprising the first 150 amino acids of amphiphysin 1 bound to both amphiphysins 1 and 2 in an overlay assay ( Fig. 2B), indicating that dimerization is mediated by this coiled-coil region of amphiphysin; this suggests the possibility that both heterodimers and homodimers are present.	bind
40395	5	10461	6	13	NULL	NULL	NULL	statement 3	Process		is					heterodimerization	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5378_821_s_65	9694653	A GST fusion protein comprising the first 150 amino acids of amphiphysin 1 bound to both amphiphysins 1 and 2 in an overlay assay ( Fig. 2B), indicating that dimerization is mediated by this coiled-coil region of amphiphysin; this suggests the possibility that both heterodimers and homodimers are present.	bind
45088	1	10461	7	NULL	NULL	0	NULL	GST fusion protein	NULL		comprise	NULL				amphiphysin 1	NULL		first 150 amino acids		NULL		0	NULL	NULL	NULL	gw60_science_281_5378_821_s_65	9694653	A GST fusion protein comprising the first 150 amino acids of amphiphysin 1 bound to both amphiphysins 1 and 2 in an overlay assay ( Fig. 2B), indicating that dimerization is mediated by this coiled-coil region of amphiphysin; this suggests the possibility that both heterodimers and homodimers are present.	bind
45089	2	10461	7	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL				amphiphysin 1	NULL				NULL		0	NULL	NULL	NULL	gw60_science_281_5378_821_s_65	9694653	A GST fusion protein comprising the first 150 amino acids of amphiphysin 1 bound to both amphiphysins 1 and 2 in an overlay assay ( Fig. 2B), indicating that dimerization is mediated by this coiled-coil region of amphiphysin; this suggests the possibility that both heterodimers and homodimers are present.	bind
45090	3	10461	7	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL				amphiphysin 2	NULL				NULL		0	NULL	NULL	NULL	gw60_science_281_5378_821_s_65	9694653	A GST fusion protein comprising the first 150 amino acids of amphiphysin 1 bound to both amphiphysins 1 and 2 in an overlay assay ( Fig. 2B), indicating that dimerization is mediated by this coiled-coil region of amphiphysin; this suggests the possibility that both heterodimers and homodimers are present.	bind
45091	4	10461	7	10	NULL	0	NULL	amphiphysin			mediates			coiled-coil region		amphiphysin 		dimerization of			NULL		NULL	NULL	NULL	NULL	gw60_science_281_5378_821_s_65	9694653	A GST fusion protein comprising the first 150 amino acids of amphiphysin 1 bound to both amphiphysins 1 and 2 in an overlay assay ( Fig. 2B), indicating that dimerization is mediated by this coiled-coil region of amphiphysin; this suggests the possibility that both heterodimers and homodimers are present.	bind
45092	5	10461	7	NULL	NULL	0	NULL	statement 2	NULL		indicate	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_science_281_5378_821_s_65	9694653	A GST fusion protein comprising the first 150 amino acids of amphiphysin 1 bound to both amphiphysins 1 and 2 in an overlay assay ( Fig. 2B), indicating that dimerization is mediated by this coiled-coil region of amphiphysin; this suggests the possibility that both heterodimers and homodimers are present.	bind
45093	6	10461	7	NULL	NULL	0	NULL	statement 3	NULL		indicate	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_science_281_5378_821_s_65	9694653	A GST fusion protein comprising the first 150 amino acids of amphiphysin 1 bound to both amphiphysins 1 and 2 in an overlay assay ( Fig. 2B), indicating that dimerization is mediated by this coiled-coil region of amphiphysin; this suggests the possibility that both heterodimers and homodimers are present.	bind
45094	7	10461	7	NULL	NULL	0	NULL	statement 5	NULL		suggests	NULL				homodimers	NULL	possibility of			NULL		0	NULL	NULL	NULL	gw60_science_281_5378_821_s_65	9694653	A GST fusion protein comprising the first 150 amino acids of amphiphysin 1 bound to both amphiphysins 1 and 2 in an overlay assay ( Fig. 2B), indicating that dimerization is mediated by this coiled-coil region of amphiphysin; this suggests the possibility that both heterodimers and homodimers are present.	bind
45095	8	10461	7	NULL	NULL	0	NULL	statement 6	NULL		suggests	NULL				heterodimers	NULL	possibility of			NULL		0	NULL	NULL	NULL	gw60_science_281_5378_821_s_65	9694653	A GST fusion protein comprising the first 150 amino acids of amphiphysin 1 bound to both amphiphysins 1 and 2 in an overlay assay ( Fig. 2B), indicating that dimerization is mediated by this coiled-coil region of amphiphysin; this suggests the possibility that both heterodimers and homodimers are present.	bind
38516	3	10462	6	13	NULL	NULL	NULL	GST-DN	GP		bind		efficiently			LIS1	GP				NULL	brain homogenates	NULL	NULL	NULL	NULL	gw60_neuron_28_3_665_s_113	11163258	A GST fusion protein containing amino acids 88-156 of mNudE (GST-DN) efficiently bound LIS1 from brain homogenates (  Figure 2B), suggesting that the LIS1 binding domain lies between amino acids 90 and 156.	bind
38517	4	10462	6	10	NULL	0	NULL		NULL		lies between	NULL		LIS1 binding domain			NULL		amino acids 90 and 156		NULL		NULL	NULL	NULL	NULL	gw60_neuron_28_3_665_s_113	11163258	A GST fusion protein containing amino acids 88-156 of mNudE (GST-DN) efficiently bound LIS1 from brain homogenates (  Figure 2B), suggesting that the LIS1 binding domain lies between amino acids 90 and 156.	bind
50196	1	10462	6	13	NULL	NULL	NULL	GST fusion protein	GP		contains					mNudE	GP		amino acids 88-156		NULL		NULL	NULL	NULL	NULL	gw60_neuron_28_3_665_s_113	11163258	A GST fusion protein containing amino acids 88-156 of mNudE (GST-DN) efficiently bound LIS1 from brain homogenates (  Figure 2B), suggesting that the LIS1 binding domain lies between amino acids 90 and 156.	bind
50197	2	10462	6	13	NULL	NULL	NULL	GST-DN	GP		is					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_28_3_665_s_113	11163258	A GST fusion protein containing amino acids 88-156 of mNudE (GST-DN) efficiently bound LIS1 from brain homogenates (  Figure 2B), suggesting that the LIS1 binding domain lies between amino acids 90 and 156.	bind
45136	1	10462	7	NULL	NULL	0	NULL	GST fusion protein	NULL		contains	NULL				mNudE	NULL		amino acids 88-156		NULL		0	NULL	NULL	NULL	gw60_neuron_28_3_665_s_113	11163258	A GST fusion protein containing amino acids 88-156 of mNudE (GST-DN) efficiently bound LIS1 from brain homogenates (  Figure 2B), suggesting that the LIS1 binding domain lies between amino acids 90 and 156.	bind
45137	2	10462	7	10	NULL	0	NULL	GST-DN	NULL		bind	NULL	efficiently			LIS1	NULL				NULL	brain homogenates	NULL	NULL	NULL	NULL	gw60_neuron_28_3_665_s_113	11163258	A GST fusion protein containing amino acids 88-156 of mNudE (GST-DN) efficiently bound LIS1 from brain homogenates (  Figure 2B), suggesting that the LIS1 binding domain lies between amino acids 90 and 156.	bind
45138	3	10462	7	NULL	NULL	0	NULL	GST-DN	NULL		is	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuron_28_3_665_s_113	11163258	A GST fusion protein containing amino acids 88-156 of mNudE (GST-DN) efficiently bound LIS1 from brain homogenates (  Figure 2B), suggesting that the LIS1 binding domain lies between amino acids 90 and 156.	bind
45139	4	10462	7	10	NULL	0	NULL		NULL		lies between	NULL		LIS1 binding domain			NULL		amino acids 90 and 156		NULL		NULL	NULL	NULL	NULL	gw60_neuron_28_3_665_s_113	11163258	A GST fusion protein containing amino acids 88-156 of mNudE (GST-DN) efficiently bound LIS1 from brain homogenates (  Figure 2B), suggesting that the LIS1 binding domain lies between amino acids 90 and 156.	bind
39074	1	10463	6	13	NULL	NULL	NULL	GST-fusion protein	GP		contains					Grb2	GP	full length			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_44_27804_s_120	9346925	A GST fusion protein containing full-length Grb2 bound HPK1 more tightly than either SH3 domain alone, indicating that the two SH3 domains of Grb2 may bind HPK1 in a bidentate fashion, as suggested by the two-hybrid analysis.	bind
39075	2	10463	6	13	NULL	NULL	NULL	statement 1	GP		bind					HPK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_44_27804_s_120	9346925	A GST fusion protein containing full-length Grb2 bound HPK1 more tightly than either SH3 domain alone, indicating that the two SH3 domains of Grb2 may bind HPK1 in a bidentate fashion, as suggested by the two-hybrid analysis.	bind
39076	3	10463	6	13	NULL	NULL	NULL	Grb2	GP		bind			SH3 domain		HPK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_44_27804_s_120	9346925	A GST fusion protein containing full-length Grb2 bound HPK1 more tightly than either SH3 domain alone, indicating that the two SH3 domains of Grb2 may bind HPK1 in a bidentate fashion, as suggested by the two-hybrid analysis.	bind
39077	4	10463	6	13	NULL	NULL	NULL	statement 2	Process		is tighter than					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_44_27804_s_120	9346925	A GST fusion protein containing full-length Grb2 bound HPK1 more tightly than either SH3 domain alone, indicating that the two SH3 domains of Grb2 may bind HPK1 in a bidentate fashion, as suggested by the two-hybrid analysis.	bind
39078	5	10463	6	13	NULL	NULL	NULL	statement 3	Process		occurs in a 					bidentate fashion	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_44_27804_s_120	9346925	A GST fusion protein containing full-length Grb2 bound HPK1 more tightly than either SH3 domain alone, indicating that the two SH3 domains of Grb2 may bind HPK1 in a bidentate fashion, as suggested by the two-hybrid analysis.	bind
45140	1	10463	7	NULL	NULL	0	NULL	GST fusion protein	NULL		contains	NULL				Grb2	NULL	full-length			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27804_s_120	9346925	A GST fusion protein containing full-length Grb2 bound HPK1 more tightly than either SH3 domain alone, indicating that the two SH3 domains of Grb2 may bind HPK1 in a bidentate fashion, as suggested by the two-hybrid analysis.	bind
45141	2	10463	7	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL	tightly			HPK1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27804_s_120	9346925	A GST fusion protein containing full-length Grb2 bound HPK1 more tightly than either SH3 domain alone, indicating that the two SH3 domains of Grb2 may bind HPK1 in a bidentate fashion, as suggested by the two-hybrid analysis.	bind
45142	3	10463	7	10	NULL	0	NULL	Grb2	NULL		bind	NULL		SH3 domain		HPK1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_44_27804_s_120	9346925	A GST fusion protein containing full-length Grb2 bound HPK1 more tightly than either SH3 domain alone, indicating that the two SH3 domains of Grb2 may bind HPK1 in a bidentate fashion, as suggested by the two-hybrid analysis.	bind
45143	4	10463	7	NULL	NULL	0	NULL	statement 2	NULL		occurs more tightly than	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27804_s_120	9346925	A GST fusion protein containing full-length Grb2 bound HPK1 more tightly than either SH3 domain alone, indicating that the two SH3 domains of Grb2 may bind HPK1 in a bidentate fashion, as suggested by the two-hybrid analysis.	bind
45144	5	10463	7	10	NULL	0	NULL	statement 3	NULL		occur in a	NULL				bidentate fashion	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_44_27804_s_120	9346925	A GST fusion protein containing full-length Grb2 bound HPK1 more tightly than either SH3 domain alone, indicating that the two SH3 domains of Grb2 may bind HPK1 in a bidentate fashion, as suggested by the two-hybrid analysis.	bind
38523	1	10464	6	13	NULL	NULL	NULL	GST fusion protein	GP		contains					CasL	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_13_6_2147_s_126	12058076	A GST fusion protein containing the CasL SH3 domain (Figure  2, lane 5) also bound efficiently to FAK, whereas GST alone failed to bind FAK (Figure  2, lane 2).	bind
38525	2	10464	6	13	NULL	NULL	NULL	statement 1	GP		bind		efficiently			FAK	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_13_6_2147_s_126	12058076	A GST fusion protein containing the CasL SH3 domain (Figure  2, lane 5) also bound efficiently to FAK, whereas GST alone failed to bind FAK (Figure  2, lane 2).	bind
38527	3	10464	6	13	NULL	NULL	NULL	GST 	GP		did not bind					FAK	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_13_6_2147_s_126	12058076	A GST fusion protein containing the CasL SH3 domain (Figure  2, lane 5) also bound efficiently to FAK, whereas GST alone failed to bind FAK (Figure  2, lane 2).	bind
45145	1	10464	7	NULL	NULL	0	NULL	GST fusion protein	NULL		contains	NULL				CasL	NULL		SH3 domain		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_13_6_2147_s_126	12058076	A GST fusion protein containing the CasL SH3 domain (Figure  2, lane 5) also bound efficiently to FAK, whereas GST alone failed to bind FAK (Figure  2, lane 2).	bind
45146	2	10464	7	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL	efficiently			FAK	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_13_6_2147_s_126	12058076	A GST fusion protein containing the CasL SH3 domain (Figure  2, lane 5) also bound efficiently to FAK, whereas GST alone failed to bind FAK (Figure  2, lane 2).	bind
45147	3	10464	7	NULL	NULL	0	NULL	GST	NULL		does not bind	NULL				FAK	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_13_6_2147_s_126	12058076	A GST fusion protein containing the CasL SH3 domain (Figure  2, lane 5) also bound efficiently to FAK, whereas GST alone failed to bind FAK (Figure  2, lane 2).	bind
38530	1	10465	6	13	NULL	NULL	NULL	Grb2	GP		bind			SH2 domain		LAT	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_24_9149_s_319	11094067	A GST fusion protein containing the SH2 domain of Grb2, which is known to bind to LAT, served as a positive control ( 73).	bind
45149	1	10465	7	10	NULL	0	NULL	Grb2	NULL		bind	NULL		SH2 domain		LAT	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_24_9149_s_319	11094067	A GST fusion protein containing the SH2 domain of Grb2, which is known to bind to LAT, served as a positive control ( 73).	bind
38545	1	10466	6	10	NULL	0	NULL		NULL		contains	NULL		236-amino acid region of the cytoplasmic tail of beta subunit			NULL		four tyrosine residues		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_26_16189_s_9	9195918	A GST fusion protein encoding a 236-amino acid region of the cytoplasmic tail of the beta subunit, which contained four tyrosine residues, bound to hck and fyn.	bind
38546	2	10466	6	13	NULL	NULL	NULL	statement 1	GP		bind					hck	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_26_16189_s_9	9195918	A GST fusion protein encoding a 236-amino acid region of the cytoplasmic tail of the beta subunit, which contained four tyrosine residues, bound to hck and fyn.	bind
38548	3	10466	6	13	NULL	NULL	NULL	statement 1	GP		bind					Fyn	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_26_16189_s_9	9195918	A GST fusion protein encoding a 236-amino acid region of the cytoplasmic tail of the beta subunit, which contained four tyrosine residues, bound to hck and fyn.	bind
45150	1	10466	7	NULL	NULL	0	NULL		NULL		contains	NULL		236-amino acid region of the cytoplasmic tail of the beta subunit			NULL		four tyrosine residues		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_26_16189_s_9	9195918	A GST fusion protein encoding a 236-amino acid region of the cytoplasmic tail of the beta subunit, which contained four tyrosine residues, bound to hck and fyn.	bind
45151	2	10466	7	NULL	NULL	0	NULL	GST fusion protein	NULL		encode	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_26_16189_s_9	9195918	A GST fusion protein encoding a 236-amino acid region of the cytoplasmic tail of the beta subunit, which contained four tyrosine residues, bound to hck and fyn.	bind
45152	3	10466	7	NULL	NULL	0	NULL	statement 2	NULL		bind	NULL				hck	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_26_16189_s_9	9195918	A GST fusion protein encoding a 236-amino acid region of the cytoplasmic tail of the beta subunit, which contained four tyrosine residues, bound to hck and fyn.	bind
45153	4	10466	7	NULL	NULL	0	NULL	statement 2	NULL		bind	NULL				fyn	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_26_16189_s_9	9195918	A GST fusion protein encoding a 236-amino acid region of the cytoplasmic tail of the beta subunit, which contained four tyrosine residues, bound to hck and fyn.	bind
38553	1	10468	6	13	NULL	NULL	NULL	Homer	GP	Drosophila	bind					mGluR5	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_4_707_s_172	9808458	A GST fusion protein of  Drosophila Homer also bound mGluR5 (data not shown).	bind
50198	2	10468	6	13	NULL	NULL	NULL	Homer	GP	Drosophila	is a type of					GST fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_21_4_707_s_172	9808458	A GST fusion protein of  Drosophila Homer also bound mGluR5 (data not shown).	bind
45154	1	10468	7	NULL	NULL	0	NULL	Homer	NULL	Drosophila	bind	NULL				mGluR5	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_21_4_707_s_172	9808458	A GST fusion protein of  Drosophila Homer also bound mGluR5 (data not shown).	bind
45155	2	10468	7	NULL	NULL	0	NULL	Homer	NULL	Drosophila	is a type of	NULL				GST fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_21_4_707_s_172	9808458	A GST fusion protein of  Drosophila Homer also bound mGluR5 (data not shown).	bind
39079	1	10469	6	13	NULL	NULL	NULL	Erk	GP		is a type of					Tyr(P)-containing protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_17_11693_s_165	10206983	A GST fusion protein of HePTP lacking this region (GST-deltaN) failed to bind any Tyr(P)-containing proteins, Erk, or p38 (Fig.  5 a) in lysates of Jurkat T cells.	bind
39080	2	10469	6	13	NULL	NULL	NULL	p38	GP		is a type of					Tyr(P)-containing protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_17_11693_s_165	10206983	A GST fusion protein of HePTP lacking this region (GST-deltaN) failed to bind any Tyr(P)-containing proteins, Erk, or p38 (Fig.  5 a) in lysates of Jurkat T cells.	bind
39081	3	10469	6	13	NULL	NULL	NULL	HePTP	GP		lacks								GST-deltaN		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_17_11693_s_165	10206983	A GST fusion protein of HePTP lacking this region (GST-deltaN) failed to bind any Tyr(P)-containing proteins, Erk, or p38 (Fig.  5 a) in lysates of Jurkat T cells.	bind
39082	4	10469	6	13	NULL	NULL	NULL	statement 3	GP		does not bind					Erk	GP				NULL	lysates of Jurkat T cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_17_11693_s_165	10206983	A GST fusion protein of HePTP lacking this region (GST-deltaN) failed to bind any Tyr(P)-containing proteins, Erk, or p38 (Fig.  5 a) in lysates of Jurkat T cells.	bind
39083	5	10469	6	13	NULL	NULL	NULL	statement 3	GP		does not bind					p38	GP				NULL	lysates of Jurkat T cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_17_11693_s_165	10206983	A GST fusion protein of HePTP lacking this region (GST-deltaN) failed to bind any Tyr(P)-containing proteins, Erk, or p38 (Fig.  5 a) in lysates of Jurkat T cells.	bind
50199	6	10469	6	13	NULL	NULL	NULL	HePTP	GP		is a type of					GST fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_17_11693_s_165	10206983	A GST fusion protein of HePTP lacking this region (GST-deltaN) failed to bind any Tyr(P)-containing proteins, Erk, or p38 (Fig.  5 a) in lysates of Jurkat T cells.	bind
45156	1	10469	7	NULL	NULL	0	NULL	HePTP	NULL		lacks	NULL					NULL		GST-deltaN		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_17_11693_s_165	10206983	A GST fusion protein of HePTP lacking this region (GST-deltaN) failed to bind any Tyr(P)-containing proteins, Erk, or p38 (Fig.  5 a) in lysates of Jurkat T cells.	bind
45157	2	10469	7	NULL	NULL	0	NULL	statement 1	NULL		does not bind	NULL				Erk	NULL				NULL	lysates of Jurkat T cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_17_11693_s_165	10206983	A GST fusion protein of HePTP lacking this region (GST-deltaN) failed to bind any Tyr(P)-containing proteins, Erk, or p38 (Fig.  5 a) in lysates of Jurkat T cells.	bind
45158	3	10469	7	NULL	NULL	0	NULL	statement 1	NULL		does not bind	NULL				p38	NULL				NULL	lysates of Jurkat T cells	0	NULL	NULL	NULL	gw60_jbiolchem_274_17_11693_s_165	10206983	A GST fusion protein of HePTP lacking this region (GST-deltaN) failed to bind any Tyr(P)-containing proteins, Erk, or p38 (Fig.  5 a) in lysates of Jurkat T cells.	bind
45159	4	10469	7	NULL	NULL	0	NULL	Erk	NULL		is a type of	NULL				Tyr(P)-containing protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_17_11693_s_165	10206983	A GST fusion protein of HePTP lacking this region (GST-deltaN) failed to bind any Tyr(P)-containing proteins, Erk, or p38 (Fig.  5 a) in lysates of Jurkat T cells.	bind
45160	5	10469	7	NULL	NULL	0	NULL	p38	NULL		is a type of	NULL				Tyr(P)-containing protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_17_11693_s_165	10206983	A GST fusion protein of HePTP lacking this region (GST-deltaN) failed to bind any Tyr(P)-containing proteins, Erk, or p38 (Fig.  5 a) in lysates of Jurkat T cells.	bind
45161	6	10469	7	NULL	NULL	0	NULL	 HePTP	NULL		is a type of	NULL				GST fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_17_11693_s_165	10206983	A GST fusion protein of HePTP lacking this region (GST-deltaN) failed to bind any Tyr(P)-containing proteins, Erk, or p38 (Fig.  5 a) in lysates of Jurkat T cells.	bind
39084	1	10470	6	13	NULL	NULL	NULL	GST-DIL	GP		bind					MBP-mADIP-F	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_6_4103_s_178	12446711	A GST fusion protein of the DIL domain of afadin (GST-DIL) bound to an MBP-fusion protein of the region of ADIP containing the all three coiled-coil domains (aa 121-436) (MBP-mADIP-F) immobilized on amylose resin beads.	bind
50203	2	10470	6	13	NULL	NULL	NULL	MBP-mADIP-F	GP		is a type of					MBP-fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_6_4103_s_178	12446711	A GST fusion protein of the DIL domain of afadin (GST-DIL) bound to an MBP-fusion protein of the region of ADIP containing the all three coiled-coil domains (aa 121-436) (MBP-mADIP-F) immobilized on amylose resin beads.	bind
50204	3	10470	6	13	NULL	NULL	NULL	MBP-mADIP-F	GP		contains					ADIP	GP		coiled-coil domains (aa 121-436)		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_6_4103_s_178	12446711	A GST fusion protein of the DIL domain of afadin (GST-DIL) bound to an MBP-fusion protein of the region of ADIP containing the all three coiled-coil domains (aa 121-436) (MBP-mADIP-F) immobilized on amylose resin beads.	bind
50205	4	10470	6	13	NULL	NULL	NULL	GST-DIL	GP		is a type of					GST fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_6_4103_s_178	12446711	A GST fusion protein of the DIL domain of afadin (GST-DIL) bound to an MBP-fusion protein of the region of ADIP containing the all three coiled-coil domains (aa 121-436) (MBP-mADIP-F) immobilized on amylose resin beads.	bind
50206	5	10470	6	13	NULL	NULL	NULL	GST-DIL	GP		contains					afadin	GP		DIL domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_6_4103_s_178	12446711	A GST fusion protein of the DIL domain of afadin (GST-DIL) bound to an MBP-fusion protein of the region of ADIP containing the all three coiled-coil domains (aa 121-436) (MBP-mADIP-F) immobilized on amylose resin beads.	bind
45162	1	10470	7	NULL	NULL	0	NULL	GST-DIL	NULL		bind	NULL				MBP-mADIP-F	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_6_4103_s_178	12446711	A GST fusion protein of the DIL domain of afadin (GST-DIL) bound to an MBP-fusion protein of the region of ADIP containing the all three coiled-coil domains (aa 121-436) (MBP-mADIP-F) immobilized on amylose resin beads.	bind
45163	2	10470	7	10	NULL	0	NULL	GST-DIL	NULL		is a type of	NULL				GST fusion protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_6_4103_s_178	12446711	A GST fusion protein of the DIL domain of afadin (GST-DIL) bound to an MBP-fusion protein of the region of ADIP containing the all three coiled-coil domains (aa 121-436) (MBP-mADIP-F) immobilized on amylose resin beads.	bind
45164	3	10470	7	10	NULL	0	NULL	MBP-mADIP-F	NULL		is a type of	NULL				MBP-fusion protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_6_4103_s_178	12446711	A GST fusion protein of the DIL domain of afadin (GST-DIL) bound to an MBP-fusion protein of the region of ADIP containing the all three coiled-coil domains (aa 121-436) (MBP-mADIP-F) immobilized on amylose resin beads.	bind
45165	4	10470	7	10	NULL	0	NULL	MBP-mADIP-F	NULL		contains	NULL				ADIP	NULL		coiled-coil domains (aa 121-436)		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_6_4103_s_178	12446711	A GST fusion protein of the DIL domain of afadin (GST-DIL) bound to an MBP-fusion protein of the region of ADIP containing the all three coiled-coil domains (aa 121-436) (MBP-mADIP-F) immobilized on amylose resin beads.	bind
50202	5	10470	7	10	NULL	0	NULL	GST-DIL	NULL		contains	NULL				afadin	NULL		DIL domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_6_4103_s_178	12446711	A GST fusion protein of the DIL domain of afadin (GST-DIL) bound to an MBP-fusion protein of the region of ADIP containing the all three coiled-coil domains (aa 121-436) (MBP-mADIP-F) immobilized on amylose resin beads.	bind
38645	1	10471	6	13	NULL	NULL	NULL	RLIP76	GP		bind		specifically	RalBD		Ral	GP	activated form of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_5_2486_s_74	9566869	A GST fusion protein of the RalBD of RLIP76 binds specifically to the activated form of Ral.	bind
50207	2	10471	6	13	NULL	NULL	NULL	RLIP76	GP		is a type of			RalBD		GST fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_5_2486_s_74	9566869	A GST fusion protein of the RalBD of RLIP76 binds specifically to the activated form of Ral.	bind
45170	1	10471	7	NULL	NULL	0	NULL	RLIP76	NULL		bind	NULL	specifically	RalBD		Ral	NULL	activated			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_5_2486_s_74	9566869	A GST fusion protein of the RalBD of RLIP76 binds specifically to the activated form of Ral.	bind
45171	2	10471	7	NULL	NULL	0	NULL	RLIP76	NULL		is a type of	NULL		RalBD		GST fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_5_2486_s_74	9566869	A GST fusion protein of the RalBD of RLIP76 binds specifically to the activated form of Ral.	bind
38646	1	10472	6	13	NULL	NULL	NULL	CED-4	GP		bind					E1B 19K	GP				NULL	yeast	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_10_6052_s_134	9742122	A GST fusion protein system was employed to confirm the binding specificity of CED-4 with E1B 19K in yeast.	bind
45172	1	10472	7	NULL	NULL	0	NULL	CED-4	NULL		bind	NULL				 E1B 19K	NULL				NULL	yeast	0	NULL	NULL	NULL	gw60_molcellbiol_18_10_6052_s_134	9742122	A GST fusion protein system was employed to confirm the binding specificity of CED-4 with E1B 19K in yeast.	bind
38647	1	10473	6	13	NULL	NULL	NULL	DPAK	GP		bind			N-terminal CRIB domain		RacA	GP	Drosophila			NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_982	10066831	A GST fusion to the DPAK N-terminal CRIB domain bound to  Drosophila RacA (DRacA) and Cdc42p (Dcdc42) and human Rac1 and Cdc42p (data not shown) in an overlay assay ( 199).	bind
38648	2	10473	6	13	NULL	NULL	NULL	DRacA	GP		is					Drosophila RacA	GP				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_982	10066831	A GST fusion to the DPAK N-terminal CRIB domain bound to  Drosophila RacA (DRacA) and Cdc42p (Dcdc42) and human Rac1 and Cdc42p (data not shown) in an overlay assay ( 199).	bind
38649	3	10473	6	13	NULL	NULL	NULL	DPAK	GP		bind			N-terminal CRIB domain		Cdc42p	GP	Drosophila			NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_982	10066831	A GST fusion to the DPAK N-terminal CRIB domain bound to  Drosophila RacA (DRacA) and Cdc42p (Dcdc42) and human Rac1 and Cdc42p (data not shown) in an overlay assay ( 199).	bind
38650	4	10473	6	13	NULL	NULL	NULL	Dcdc42	GP		is					Drosophila Cdc42p	GP				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_982	10066831	A GST fusion to the DPAK N-terminal CRIB domain bound to  Drosophila RacA (DRacA) and Cdc42p (Dcdc42) and human Rac1 and Cdc42p (data not shown) in an overlay assay ( 199).	bind
38651	5	10473	6	13	NULL	NULL	NULL	DPAK	GP		bind			N-terminal CRIB domain		Rac1	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_982	10066831	A GST fusion to the DPAK N-terminal CRIB domain bound to  Drosophila RacA (DRacA) and Cdc42p (Dcdc42) and human Rac1 and Cdc42p (data not shown) in an overlay assay ( 199).	bind
38652	6	10473	6	13	NULL	NULL	NULL	DPAK	GP		bind			N-terminal CRIB domain		Cdc42p	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_982	10066831	A GST fusion to the DPAK N-terminal CRIB domain bound to  Drosophila RacA (DRacA) and Cdc42p (Dcdc42) and human Rac1 and Cdc42p (data not shown) in an overlay assay ( 199).	bind
45173	1	10473	7	NULL	NULL	0	NULL	DPAK	NULL		bind	NULL		N-terminal CRIB domain		DRacA	NULL				NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_982	10066831	A GST fusion to the DPAK N-terminal CRIB domain bound to  Drosophila RacA (DRacA) and Cdc42p (Dcdc42) and human Rac1 and Cdc42p (data not shown) in an overlay assay ( 199).	bind
45174	2	10473	7	NULL	NULL	0	NULL	DPAK	NULL		bind	NULL		N-terminal CRIB domain		Dcdc42	NULL				NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_982	10066831	A GST fusion to the DPAK N-terminal CRIB domain bound to  Drosophila RacA (DRacA) and Cdc42p (Dcdc42) and human Rac1 and Cdc42p (data not shown) in an overlay assay ( 199).	bind
45175	3	10473	7	NULL	NULL	0	NULL	DPAK	NULL		bind	NULL		N-terminal CRIB domain		Rac1	NULL	human			NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_982	10066831	A GST fusion to the DPAK N-terminal CRIB domain bound to  Drosophila RacA (DRacA) and Cdc42p (Dcdc42) and human Rac1 and Cdc42p (data not shown) in an overlay assay ( 199).	bind
45176	4	10473	7	NULL	NULL	0	NULL	DPAK	NULL		bind	NULL		N-terminal CRIB domain		Cdc42p	NULL	human			NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_982	10066831	A GST fusion to the DPAK N-terminal CRIB domain bound to  Drosophila RacA (DRacA) and Cdc42p (Dcdc42) and human Rac1 and Cdc42p (data not shown) in an overlay assay ( 199).	bind
45177	5	10473	7	10	NULL	0	NULL	DRacA			is					Drosophila RacA					NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_982	10066831	A GST fusion to the DPAK N-terminal CRIB domain bound to  Drosophila RacA (DRacA) and Cdc42p (Dcdc42) and human Rac1 and Cdc42p (data not shown) in an overlay assay ( 199).	bind
45178	6	10473	7	10	NULL	0	NULL	Dcdc42			is					Drosophila Cdc42p					NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_982	10066831	A GST fusion to the DPAK N-terminal CRIB domain bound to  Drosophila RacA (DRacA) and Cdc42p (Dcdc42) and human Rac1 and Cdc42p (data not shown) in an overlay assay ( 199).	bind
38653	1	10474	6	13	NULL	NULL	NULL	Sp1-F	GP		bind					huntington	GP	transfected			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_5_1277_s_151	11839795	A GST pull down assay showed that Sp1-F and Sp1-C bound to transfected huntingtin, whereas Sp1-P or Sp1-N did not (Fig.  1C).	bind
38654	2	10474	6	13	NULL	NULL	NULL	Sp1-C	GP		bind					huntington	GP	transfected			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_5_1277_s_151	11839795	A GST pull down assay showed that Sp1-F and Sp1-C bound to transfected huntingtin, whereas Sp1-P or Sp1-N did not (Fig.  1C).	bind
38655	3	10474	6	13	NULL	NULL	NULL	Sp1-P	GP		does not bind					huntington	GP	transfected			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_5_1277_s_151	11839795	A GST pull down assay showed that Sp1-F and Sp1-C bound to transfected huntingtin, whereas Sp1-P or Sp1-N did not (Fig.  1C).	bind
38656	4	10474	6	13	NULL	NULL	NULL	Sp1-N	GP		does not bind					huntington	GP	transfected			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_5_1277_s_151	11839795	A GST pull down assay showed that Sp1-F and Sp1-C bound to transfected huntingtin, whereas Sp1-P or Sp1-N did not (Fig.  1C).	bind
45180	1	10474	7	NULL	NULL	0	NULL	Sp1-F	NULL		bind	NULL				 huntingtin	NULL	transfected			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_5_1277_s_151	11839795	A GST pull down assay showed that Sp1-F and Sp1-C bound to transfected huntingtin, whereas Sp1-P or Sp1-N did not (Fig.  1C).	bind
45181	2	10474	7	NULL	NULL	0	NULL	Sp1-C	NULL		bind	NULL				huntingtin	NULL	transfected			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_5_1277_s_151	11839795	A GST pull down assay showed that Sp1-F and Sp1-C bound to transfected huntingtin, whereas Sp1-P or Sp1-N did not (Fig.  1C).	bind
45182	3	10474	7	NULL	NULL	0	NULL	Sp1-P	NULL		does not bind	NULL				huntingtin	NULL	transfected			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_5_1277_s_151	11839795	A GST pull down assay showed that Sp1-F and Sp1-C bound to transfected huntingtin, whereas Sp1-P or Sp1-N did not (Fig.  1C).	bind
45183	4	10474	7	NULL	NULL	0	NULL	Sp1-N	NULL		does not bind	NULL				huntingtin	NULL	transfected			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_5_1277_s_151	11839795	A GST pull down assay showed that Sp1-F and Sp1-C bound to transfected huntingtin, whereas Sp1-P or Sp1-N did not (Fig.  1C).	bind
38657	1	10475	6	13	NULL	NULL	NULL	HCF	GP		bind					ZF	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_12_2446_s_183	10871379	A GST pull-down assay (Fig.  4B) and a mammalian two-hybrid assay (Fig.  4C) were performed to examine the effects of these mutations on the  in vitro as well as  in vivo binding of HCF by ZF.	bind
38658	2	10475	6	13	NULL	NULL	NULL	HCF	GP		bind					ZF	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_12_2446_s_183	10871379	A GST pull-down assay (Fig.  4B) and a mammalian two-hybrid assay (Fig.  4C) were performed to examine the effects of these mutations on the  in vitro as well as  in vivo binding of HCF by ZF.	bind
45184	1	10475	7	10	NULL	0	NULL	ZF	NULL		bind	NULL				HCF	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_12_2446_s_183	10871379	A GST pull-down assay (Fig.  4B) and a mammalian two-hybrid assay (Fig.  4C) were performed to examine the effects of these mutations on the  in vitro as well as  in vivo binding of HCF by ZF.	bind
50208	2	10475	7	10	NULL	0	NULL	ZF	NULL		bind	NULL				HCF	NULL				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_12_2446_s_183	10871379	A GST pull-down assay (Fig.  4B) and a mammalian two-hybrid assay (Fig.  4C) were performed to examine the effects of these mutations on the  in vitro as well as  in vivo binding of HCF by ZF.	bind
38659	1	10476	6	13	NULL	NULL	NULL	bZIP	GP	radiolabeled	bind								gst-DBD		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_50_41421_s_113	16223730	A GST pull-down assay demonstrating binding of radiolabled bZIP or IE2 probe to gst-DBD  with the indicated substitutions at Arg232 and Arg235 is shown.	bind
38660	2	10476	6	13	NULL	NULL	NULL	IE2 probe	GP		bind								gst-DBD		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_50_41421_s_113	16223730	A GST pull-down assay demonstrating binding of radiolabled bZIP or IE2 probe to gst-DBD  with the indicated substitutions at Arg232 and Arg235 is shown.	bind
45185	1	10476	7	10	NULL	0	NULL	bZIP		radiolabeled 	bind								gst-DBD		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_50_41421_s_113	16223730	A GST pull-down assay demonstrating binding of radiolabled bZIP or IE2 probe to gst-DBD  with the indicated substitutions at Arg232 and Arg235 is shown.	bind
45187	2	10476	7	10	NULL	0	NULL	IE2 probe			bind								gst-DBD		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_50_41421_s_113	16223730	A GST pull-down assay demonstrating binding of radiolabled bZIP or IE2 probe to gst-DBD  with the indicated substitutions at Arg232 and Arg235 is shown.	bind
38661	1	10477	6	13	NULL	NULL	NULL	His6-KRAB-A	GP	35S-labeled	bind		specifically			GST-pVHL19	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_22_8_1857_s_106	12682018	A GST pull-down assay result further demonstrated that the 35S-labeled His6-KRAB-A specifically bound to the GST - pVHL19 fusion protein, but not to GST alone (Figure  2F), indicating a physical association  in vitro.	bind
50209	2	10477	6	13	NULL	NULL	NULL	GST-pVHL19	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_8_1857_s_106	12682018	A GST pull-down assay result further demonstrated that the 35S-labeled His6-KRAB-A specifically bound to the GST - pVHL19 fusion protein, but not to GST alone (Figure  2F), indicating a physical association  in vitro.	bind
50210	3	10477	6	13	NULL	NULL	NULL	His6-KRAB-A \t	GP	35S-labeled	does not bind					GST	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_8_1857_s_106	12682018	A GST pull-down assay result further demonstrated that the 35S-labeled His6-KRAB-A specifically bound to the GST - pVHL19 fusion protein, but not to GST alone (Figure  2F), indicating a physical association  in vitro.	bind
45189	1	10477	7	NULL	NULL	0	NULL	His6-KRAB-A	NULL	 35S-labeled	bind	NULL	specifically			GST - pVHL19	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_embo_22_8_1857_s_106	12682018	A GST pull-down assay result further demonstrated that the 35S-labeled His6-KRAB-A specifically bound to the GST - pVHL19 fusion protein, but not to GST alone (Figure  2F), indicating a physical association  in vitro.	bind
45190	2	10477	7	NULL	NULL	0	NULL	His6-KRAB-A	NULL	35S-labeled	does not bind	NULL	 			GST	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_22_8_1857_s_106	12682018	A GST pull-down assay result further demonstrated that the 35S-labeled His6-KRAB-A specifically bound to the GST - pVHL19 fusion protein, but not to GST alone (Figure  2F), indicating a physical association  in vitro.	bind
45191	3	10477	7	NULL	NULL	0	NULL	GST - pVHL19	NULL		is a type of	NULL				GST fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_22_8_1857_s_106	12682018	A GST pull-down assay result further demonstrated that the 35S-labeled His6-KRAB-A specifically bound to the GST - pVHL19 fusion protein, but not to GST alone (Figure  2F), indicating a physical association  in vitro.	bind
39087	1	10479	6	13	NULL	NULL	NULL	N-CoR	GP		bind		directly	ID1		ERalpha	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_233	12738788	A GST pull-down assay showed both  GST-ID1-2 derived from N-CoR and SMRT directly bound to ERalpha in the  presence of OHT ( Fig.  6 B).	bind
39088	2	10479	6	13	NULL	NULL	NULL	N-CoR	GP		bind		directly	ID2		ERalpha	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_233	12738788	A GST pull-down assay showed both  GST-ID1-2 derived from N-CoR and SMRT directly bound to ERalpha in the  presence of OHT ( Fig.  6 B).	bind
39089	3	10479	6	13	NULL	NULL	NULL	SMRT	GP		bind		directly	ID1		ERalpha	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_233	12738788	A GST pull-down assay showed both  GST-ID1-2 derived from N-CoR and SMRT directly bound to ERalpha in the  presence of OHT ( Fig.  6 B).	bind
39090	4	10479	6	13	NULL	NULL	NULL	SMRT	GP		bind		directly	ID2		ERalpha	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_233	12738788	A GST pull-down assay showed both  GST-ID1-2 derived from N-CoR and SMRT directly bound to ERalpha in the  presence of OHT ( Fig.  6 B).	bind
39091	5	10479	6	13	NULL	NULL	NULL	statement 1	Process		occurs in presence of					OHT	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_233	12738788	A GST pull-down assay showed both  GST-ID1-2 derived from N-CoR and SMRT directly bound to ERalpha in the  presence of OHT ( Fig.  6 B).	bind
39092	6	10479	6	13	NULL	NULL	NULL	statement 2	Process		occurs in presence of					OHT	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_233	12738788	A GST pull-down assay showed both  GST-ID1-2 derived from N-CoR and SMRT directly bound to ERalpha in the  presence of OHT ( Fig.  6 B).	bind
39093	7	10479	6	13	NULL	NULL	NULL	statement 3	Process		occurs in presence of					OHT	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_233	12738788	A GST pull-down assay showed both  GST-ID1-2 derived from N-CoR and SMRT directly bound to ERalpha in the  presence of OHT ( Fig.  6 B).	bind
39094	8	10479	6	13	NULL	NULL	NULL	statement 4	Process		occurs in presence of					OHT	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_233	12738788	A GST pull-down assay showed both  GST-ID1-2 derived from N-CoR and SMRT directly bound to ERalpha in the  presence of OHT ( Fig.  6 B).	bind
45192	1	10479	7	10	NULL	0	NULL	N-CoR			bind		directly	ID1		ERalpha					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_233	12738788	A GST pull-down assay showed both  GST-ID1-2 derived from N-CoR and SMRT directly bound to ERalpha in the  presence of OHT ( Fig.  6 B).	bind
45193	2	10479	7	10	NULL	0	NULL	N-CoR			bind		directly	ID2		ERalpha					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_233	12738788	A GST pull-down assay showed both  GST-ID1-2 derived from N-CoR and SMRT directly bound to ERalpha in the  presence of OHT ( Fig.  6 B).	bind
45194	3	10479	7	10	NULL	0	NULL	SMRT			bind		directly	ID1		ERalpha					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_233	12738788	A GST pull-down assay showed both  GST-ID1-2 derived from N-CoR and SMRT directly bound to ERalpha in the  presence of OHT ( Fig.  6 B).	bind
45195	4	10479	7	10	NULL	0	NULL	SMRT			bind		directly	ID2		ERalpha					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_233	12738788	A GST pull-down assay showed both  GST-ID1-2 derived from N-CoR and SMRT directly bound to ERalpha in the  presence of OHT ( Fig.  6 B).	bind
45196	5	10479	7	10	NULL	0	NULL	statement 1			in the presence of					OHT					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_233	12738788	A GST pull-down assay showed both  GST-ID1-2 derived from N-CoR and SMRT directly bound to ERalpha in the  presence of OHT ( Fig.  6 B).	bind
57618	6	10479	7	10	NULL	0	NULL	statement 2			in the presence of					OHT					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_233	12738788	A GST pull-down assay showed both  GST-ID1-2 derived from N-CoR and SMRT directly bound to ERalpha in the  presence of OHT ( Fig.  6 B).	bind
57619	7	10479	7	10	NULL	0	NULL	statement 3			in the presence of					OHT					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_233	12738788	A GST pull-down assay showed both  GST-ID1-2 derived from N-CoR and SMRT directly bound to ERalpha in the  presence of OHT ( Fig.  6 B).	bind
57620	8	10479	7	10	NULL	0	NULL	statement 4			in the presence of					statement 8					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_233	12738788	A GST pull-down assay showed both  GST-ID1-2 derived from N-CoR and SMRT directly bound to ERalpha in the  presence of OHT ( Fig.  6 B).	bind
38913	1	10480	6	13	NULL	NULL	NULL	FOXO1	GP	in vitro-translated	bind					GST-mPXR	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_18_7931_s_210	15340055	A GST pull-down assay showed that in vitro-translated FOXO1 bound to GST-mPXR, which was increased by the specific PXR activator pregnenolone PCN (Fig.  6a).	bind
38914	2	10480	6	13	NULL	NULL	NULL	PCN	Chemical		increases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_18_7931_s_210	15340055	A GST pull-down assay showed that in vitro-translated FOXO1 bound to GST-mPXR, which was increased by the specific PXR activator pregnenolone PCN (Fig.  6a).	bind
38915	3	10480	6	13	NULL	NULL	NULL	PCN	Chemical		is a type of					PXR activator	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_18_7931_s_210	15340055	A GST pull-down assay showed that in vitro-translated FOXO1 bound to GST-mPXR, which was increased by the specific PXR activator pregnenolone PCN (Fig.  6a).	bind
50211	4	10480	6	13	NULL	NULL	NULL	PCN	Chemical		is					pregnenolone	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_18_7931_s_210	15340055	A GST pull-down assay showed that in vitro-translated FOXO1 bound to GST-mPXR, which was increased by the specific PXR activator pregnenolone PCN (Fig.  6a).	bind
45197	1	10480	7	NULL	NULL	0	NULL	FOXO1	NULL	in vitro-translated	bind	NULL				GST-mPXR	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_18_7931_s_210	15340055	A GST pull-down assay showed that in vitro-translated FOXO1 bound to GST-mPXR, which was increased by the specific PXR activator pregnenolone PCN (Fig.  6a).	bind
45198	2	10480	7	10	NULL	0	NULL	PCN	NULL		increase	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_18_7931_s_210	15340055	A GST pull-down assay showed that in vitro-translated FOXO1 bound to GST-mPXR, which was increased by the specific PXR activator pregnenolone PCN (Fig.  6a).	bind
45199	3	10480	7	10	NULL	0	NULL	PCN	NULL		is a type of	NULL				PXR activator	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_18_7931_s_210	15340055	A GST pull-down assay showed that in vitro-translated FOXO1 bound to GST-mPXR, which was increased by the specific PXR activator pregnenolone PCN (Fig.  6a).	bind
50212	4	10480	7	10	NULL	0	NULL	PCN	NULL		is	NULL				pregnenolone	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_18_7931_s_210	15340055	A GST pull-down assay showed that in vitro-translated FOXO1 bound to GST-mPXR, which was increased by the specific PXR activator pregnenolone PCN (Fig.  6a).	bind
38916	1	10481	6	13	NULL	NULL	NULL	TaWIN1	GP		bind		specifically;;directly			GST-WPK4	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_31695_s_84	10918058	A GST pull-down assay showed that TaWIN1 specifically binds GST-WPK4 but not GST-K75D  in vitro, indicating a direct interaction between WPK4 and TaWIN1 Fig.  2 C).	bind
38917	2	10481	6	13	NULL	NULL	NULL	TaWIN1	GP		does not bind								GST-K75D		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_31695_s_84	10918058	A GST pull-down assay showed that TaWIN1 specifically binds GST-WPK4 but not GST-K75D  in vitro, indicating a direct interaction between WPK4 and TaWIN1 Fig.  2 C).	bind
45202	1	10481	7	NULL	NULL	0	NULL	TaWIN1	NULL		bind	NULL	specifically;;directly			GST-WPK4	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_31695_s_84	10918058	A GST pull-down assay showed that TaWIN1 specifically binds GST-WPK4 but not GST-K75D  in vitro, indicating a direct interaction between WPK4 and TaWIN1 Fig.  2 C).	bind
45203	2	10481	7	NULL	NULL	0	NULL	TaWIN1 	NULL		does not bind	NULL					NULL		GST-K75D		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_31695_s_84	10918058	A GST pull-down assay showed that TaWIN1 specifically binds GST-WPK4 but not GST-K75D  in vitro, indicating a direct interaction between WPK4 and TaWIN1 Fig.  2 C).	bind
39095	1	10482	6	13	NULL	NULL	NULL	SRC-1	GP		is a type of					AF-2 coactivator	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
39096	2	10482	6	13	NULL	NULL	NULL	TRAP220	GP		is a type of					AF-2 coactivator	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
39097	3	10482	6	13	NULL	NULL	NULL	TRRAP	GP		is a type of					AF-2 coactivator	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
39098	4	10482	6	13	NULL	NULL	NULL	ERalpha(GAL-DEF)	GP		bind		directly			SRC-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
39099	5	10482	6	13	NULL	NULL	NULL	ERalpha(GAL-DEF)	GP		bind		directly			TRAP220	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
39100	6	10482	6	13	NULL	NULL	NULL	ERalpha(GAL-DEF)	GP		bind		directly			TRRAP	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
39101	7	10482	6	13	NULL	NULL	NULL	E2	Chemical		induces					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
39102	8	10482	6	13	NULL	NULL	NULL	E2	Chemical		induces					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
39103	9	10482	6	13	NULL	NULL	NULL	E2	Chemical		induces					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
39104	10	10482	6	13	NULL	NULL	NULL	BBP	Chemical		abrogates					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
39105	11	10482	6	13	NULL	NULL	NULL	BBP	Chemical		abrogates					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
39106	12	10482	6	13	NULL	NULL	NULL	BBP	Chemical		abrogates					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
39107	13	10482	6	13	NULL	NULL	NULL	OHT	Chemical		abrogates					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
39108	14	10482	6	13	NULL	NULL	NULL	OHT	Chemical		abrogates					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
39109	15	10482	6	13	NULL	NULL	NULL	OHT	Chemical		abrogates					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
45207	1	10482	7	NULL	NULL	0	NULL	ERalpha	NULL		bind	NULL	directly			SRC-1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
45223	2	10482	7	NULL	NULL	0	NULL	ERalpha	NULL		bind	NULL	directly			TRAP220	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
45225	3	10482	7	NULL	NULL	0	NULL	ERalpha	NULL		bind	NULL	directly			TRRAP	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
45228	4	10482	7	NULL	NULL	0	NULL	E2	NULL		induce	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
45229	5	10482	7	NULL	NULL	0	NULL	E2	NULL		induce	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
45230	6	10482	7	NULL	NULL	0	NULL	E2	NULL		induce	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
45236	7	10482	7	NULL	NULL	0	NULL	statement 2	NULL		is an alternative to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
45240	8	10482	7	NULL	NULL	0	NULL	BBP 	NULL		abrogates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
45242	9	10482	7	NULL	NULL	0	NULL	BBP	NULL		abrogates	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
45244	10	10482	7	NULL	NULL	0	NULL	BBP	NULL		abrogates	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
45245	11	10482	7	NULL	NULL	0	NULL	OHT	NULL		abrogates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
45248	12	10482	7	NULL	NULL	0	NULL	OHT	NULL		abrogates	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
45249	13	10482	7	NULL	NULL	0	NULL	OHT	NULL		abrogates	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
45251	14	10482	7	NULL	NULL	0	NULL	ERalpha	NULL		is	NULL				GAL-DEF	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
45252	15	10482	7	NULL	NULL	0	NULL	SRC-1	NULL		is a type of	NULL				AF-2 coactivator	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
45253	16	10482	7	NULL	NULL	0	NULL	TRAP220	NULL		is a type of	NULL				AF-2 coactivator	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
45255	17	10482	7	NULL	NULL	0	NULL	TRRAP	NULL		is a type of	NULL				AF-2 coactivator	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_29_26704_s_171	12738788	A GST pull-down assay showed that whereas E2 induced the direct  binding of ERalpha(GAL-DEF) to AF-2 coactivators SRC-1, TRAP220, or TRRAP,  BBP and OHT abrogated the interaction between GAL-DEF and AF-2 coactivators  ( Fig. 3 C).	bind
38918	1	10483	6	13	NULL	NULL	NULL	cdr2	GP		bind					c-Myc	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_genesdev_13_16_2087_s_45	10465786	A GST pull-down assay was used to examine the in vitro binding of cdr2 and c-Myc.	bind
45261	1	10483	7	NULL	NULL	0	NULL	cdr2	NULL		bind	NULL				c-Myc	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_genesdev_13_16_2087_s_45	10465786	A GST pull-down assay was used to examine the in vitro binding of cdr2 and c-Myc.	bind
38919	1	10484	6	13	NULL	NULL	NULL	CtBP protein	GP	GAL4-tagged	bind					GST-MLL	GP	immobilized	R/MT		NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_14_8342_s_108	12829790	A GST pull-down assay with various, immobilized GST-MLL RD  proteins incubated with GAL4-tagged CtBP protein expressed by transient  transfection demonstrated that CtBP binds to both MLL(R/MT) and MLL(RD1) but  not to GST alone or to MLL(RD2) ( Fig.  4 A).	bind
38920	2	10484	6	13	NULL	NULL	NULL	CtBP protein	GP	GAL4-tagged	bind					GST-MLL	GP	immobilized	RD1		NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_14_8342_s_108	12829790	A GST pull-down assay with various, immobilized GST-MLL RD  proteins incubated with GAL4-tagged CtBP protein expressed by transient  transfection demonstrated that CtBP binds to both MLL(R/MT) and MLL(RD1) but  not to GST alone or to MLL(RD2) ( Fig.  4 A).	bind
38921	3	10484	6	13	NULL	NULL	NULL	CtBP protein	GP	GAL4-tagged	does not bind					GST-MLL	GP	immobilized	RD2		NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_14_8342_s_108	12829790	A GST pull-down assay with various, immobilized GST-MLL RD  proteins incubated with GAL4-tagged CtBP protein expressed by transient  transfection demonstrated that CtBP binds to both MLL(R/MT) and MLL(RD1) but  not to GST alone or to MLL(RD2) ( Fig.  4 A).	bind
50217	4	10484	6	13	NULL	NULL	NULL	CtBP protein	GP	GAL4-tagged	does not bind					GST	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_14_8342_s_108	12829790	A GST pull-down assay with various, immobilized GST-MLL RD  proteins incubated with GAL4-tagged CtBP protein expressed by transient  transfection demonstrated that CtBP binds to both MLL(R/MT) and MLL(RD1) but  not to GST alone or to MLL(RD2) ( Fig.  4 A).	bind
45278	1	10484	7	10	NULL	0	NULL	CtBP protein	NULL	GAL4-tagged	bind	NULL				GST-MLL	NULL	immobilized	R/MT		NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_14_8342_s_108	12829790	A GST pull-down assay with various, immobilized GST-MLL RD  proteins incubated with GAL4-tagged CtBP protein expressed by transient  transfection demonstrated that CtBP binds to both MLL(R/MT) and MLL(RD1) but  not to GST alone or to MLL(RD2) ( Fig.  4 A).	bind
45282	2	10484	7	10	NULL	0	NULL	CtBP protein	NULL	GAL4-tagged	bind	NULL				GST-MLL	NULL	immobilized	RD1		NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_14_8342_s_108	12829790	A GST pull-down assay with various, immobilized GST-MLL RD  proteins incubated with GAL4-tagged CtBP protein expressed by transient  transfection demonstrated that CtBP binds to both MLL(R/MT) and MLL(RD1) but  not to GST alone or to MLL(RD2) ( Fig.  4 A).	bind
45285	3	10484	7	NULL	NULL	0	NULL	CtBP protein	NULL	GAL4-tagged	does not bind	NULL				GST	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_100_14_8342_s_108	12829790	A GST pull-down assay with various, immobilized GST-MLL RD  proteins incubated with GAL4-tagged CtBP protein expressed by transient  transfection demonstrated that CtBP binds to both MLL(R/MT) and MLL(RD1) but  not to GST alone or to MLL(RD2) ( Fig.  4 A).	bind
45286	4	10484	7	10	NULL	0	NULL	CtBP protein	NULL	GAL4-tagged	does not bind	NULL				GST-MLL	NULL	immobilized	RD2		NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_14_8342_s_108	12829790	A GST pull-down assay with various, immobilized GST-MLL RD  proteins incubated with GAL4-tagged CtBP protein expressed by transient  transfection demonstrated that CtBP binds to both MLL(R/MT) and MLL(RD1) but  not to GST alone or to MLL(RD2) ( Fig.  4 A).	bind
39110	1	10486	6	13	NULL	NULL	NULL	gp185ErbB-2	GP		bind					GST-clone 52	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_20_7735_s_124	11003669	A GST-clone 52 fusion protein readily bound constitutively active gp185ErbB-2 (Fig.  1B) solubilized from NIH-ErbB-2 transfectants ( 17), whereas no ErbB-2 binding to GST beads (Fig.  1B) and GST-clone 52 beads incubated with NIH 3T3 lysates (data not shown) was observed.	bind
39113	2	10486	6	13	NULL	NULL	NULL	ErbB-2	GP		does not bind					GST-clone 52	GP				NULL	NIH 3T3 lysates	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_20_7735_s_124	11003669	A GST-clone 52 fusion protein readily bound constitutively active gp185ErbB-2 (Fig.  1B) solubilized from NIH-ErbB-2 transfectants ( 17), whereas no ErbB-2 binding to GST beads (Fig.  1B) and GST-clone 52 beads incubated with NIH 3T3 lysates (data not shown) was observed.	bind
50218	3	10486	6	13	NULL	NULL	NULL	GST-clone 52	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_20_7735_s_124	11003669	A GST-clone 52 fusion protein readily bound constitutively active gp185ErbB-2 (Fig.  1B) solubilized from NIH-ErbB-2 transfectants ( 17), whereas no ErbB-2 binding to GST beads (Fig.  1B) and GST-clone 52 beads incubated with NIH 3T3 lysates (data not shown) was observed.	bind
50219	4	10486	6	13	NULL	NULL	NULL	ErbB-2	GP		does not bind					GST	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_20_7735_s_124	11003669	A GST-clone 52 fusion protein readily bound constitutively active gp185ErbB-2 (Fig.  1B) solubilized from NIH-ErbB-2 transfectants ( 17), whereas no ErbB-2 binding to GST beads (Fig.  1B) and GST-clone 52 beads incubated with NIH 3T3 lysates (data not shown) was observed.	bind
45368	2	10486	7	NULL	NULL	0	NULL	GST-clone 52 protein	NULL		bind	NULL	readily			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_20_7735_s_124	11003669	A GST-clone 52 fusion protein readily bound constitutively active gp185ErbB-2 (Fig.  1B) solubilized from NIH-ErbB-2 transfectants ( 17), whereas no ErbB-2 binding to GST beads (Fig.  1B) and GST-clone 52 beads incubated with NIH 3T3 lysates (data not shown) was observed.	bind
45369	1	10486	7	NULL	NULL	0	NULL	gp185ErbB-2	NULL		is solubilized from	NULL				NIH-ErbB-2 transfectants	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_20_7735_s_124	11003669	A GST-clone 52 fusion protein readily bound constitutively active gp185ErbB-2 (Fig.  1B) solubilized from NIH-ErbB-2 transfectants ( 17), whereas no ErbB-2 binding to GST beads (Fig.  1B) and GST-clone 52 beads incubated with NIH 3T3 lysates (data not shown) was observed.	bind
45370	3	10486	7	10	NULL	0	NULL	 ErbB-2	NULL		does not bind	NULL				GST	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_20_7735_s_124	11003669	A GST-clone 52 fusion protein readily bound constitutively active gp185ErbB-2 (Fig.  1B) solubilized from NIH-ErbB-2 transfectants ( 17), whereas no ErbB-2 binding to GST beads (Fig.  1B) and GST-clone 52 beads incubated with NIH 3T3 lysates (data not shown) was observed.	bind
45371	4	10486	7	NULL	NULL	0	NULL	ErbB-2	NULL		does not bind	NULL				GST-clone 52	NULL				NULL	NIH 3T3 lysates 	0	NULL	NULL	NULL	gw60_molcellbiol_20_20_7735_s_124	11003669	A GST-clone 52 fusion protein readily bound constitutively active gp185ErbB-2 (Fig.  1B) solubilized from NIH-ErbB-2 transfectants ( 17), whereas no ErbB-2 binding to GST beads (Fig.  1B) and GST-clone 52 beads incubated with NIH 3T3 lysates (data not shown) was observed.	bind
45372	5	10486	7	NULL	NULL	0	NULL	GST-clone 52	NULL		is a type of	NULL				fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_20_7735_s_124	11003669	A GST-clone 52 fusion protein readily bound constitutively active gp185ErbB-2 (Fig.  1B) solubilized from NIH-ErbB-2 transfectants ( 17), whereas no ErbB-2 binding to GST beads (Fig.  1B) and GST-clone 52 beads incubated with NIH 3T3 lysates (data not shown) was observed.	bind
38929	1	10487	6	13	NULL	NULL	NULL	GST-CRIB	GP	immobilized	bind					GFP-Cdc42	GP				NULL	yeast lysates	NULL	NULL	NULL	NULL	gw70_pnas_103_11_4116_s_152	16537494	A GST-CRIB fusion protein immobilized on glutathione beads was incubated with yeast lysates; bound GFP-Cdc42.	bind
50220	2	10487	6	13	NULL	NULL	NULL	GST-CRIB	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_11_4116_s_152	16537494	A GST-CRIB fusion protein immobilized on glutathione beads was incubated with yeast lysates; bound GFP-Cdc42.	bind
45373	1	10487	7	NULL	NULL	0	NULL	GST-CRIB protein	NULL	immobilized	bind	NULL				GFP-Cdc42	NULL				NULL	yeast lysates	0	NULL	NULL	NULL	gw70_pnas_103_11_4116_s_152	16537494	A GST-CRIB fusion protein immobilized on glutathione beads was incubated with yeast lysates; bound GFP-Cdc42.	bind
45374	2	10487	7	NULL	NULL	0	NULL	GST-CRIB protein	NULL		is a type of	NULL				fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_103_11_4116_s_152	16537494	A GST-CRIB fusion protein immobilized on glutathione beads was incubated with yeast lysates; bound GFP-Cdc42.	bind
38930	1	10488	6	13	NULL	NULL	NULL	GST-Ebp1	GP		encodes								amino acids 293 - 372		NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_8_2168_s_197	12682367	A GST-Ebp1 fusion protein encoding amino acids 293 - 372 (encompassing the HDAC2 binding domain) bound HDAC enzymatic activity as well as full-length Ebp1.	bind
38931	2	10488	6	13	NULL	NULL	NULL	GST-Ebp1	GP		encompasses								HDAC2 binding domain		NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_8_2168_s_197	12682367	A GST-Ebp1 fusion protein encoding amino acids 293 - 372 (encompassing the HDAC2 binding domain) bound HDAC enzymatic activity as well as full-length Ebp1.	bind
38932	3	10488	6	13	NULL	NULL	NULL	GST-Ebp1	GP		bind					HDAC	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_8_2168_s_197	12682367	A GST-Ebp1 fusion protein encoding amino acids 293 - 372 (encompassing the HDAC2 binding domain) bound HDAC enzymatic activity as well as full-length Ebp1.	bind
38933	4	10488	6	13	NULL	NULL	NULL	GST-Ebp1	GP		bind					Ebp1	GP	full length			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_8_2168_s_197	12682367	A GST-Ebp1 fusion protein encoding amino acids 293 - 372 (encompassing the HDAC2 binding domain) bound HDAC enzymatic activity as well as full-length Ebp1.	bind
50221	5	10488	6	13	NULL	NULL	NULL	GST-Ebp1 	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_8_2168_s_197	12682367	A GST-Ebp1 fusion protein encoding amino acids 293 - 372 (encompassing the HDAC2 binding domain) bound HDAC enzymatic activity as well as full-length Ebp1.	bind
45375	1	10488	7	NULL	NULL	0	NULL	GST-Ebp1	NULL		encode	NULL					NULL		amino acids 293 - 372		NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_8_2168_s_197	12682367	A GST-Ebp1 fusion protein encoding amino acids 293 - 372 (encompassing the HDAC2 binding domain) bound HDAC enzymatic activity as well as full-length Ebp1.	bind
45376	2	10488	7	10	NULL	0	NULL	statement 1			encompass								HDAC2 binding domain		NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_8_2168_s_197	12682367	A GST-Ebp1 fusion protein encoding amino acids 293 - 372 (encompassing the HDAC2 binding domain) bound HDAC enzymatic activity as well as full-length Ebp1.	bind
45377	3	10488	7	NULL	NULL	0	NULL	statement 2	NULL		bind	NULL				HDAC	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_8_2168_s_197	12682367	A GST-Ebp1 fusion protein encoding amino acids 293 - 372 (encompassing the HDAC2 binding domain) bound HDAC enzymatic activity as well as full-length Ebp1.	bind
45378	4	10488	7	NULL	NULL	0	NULL	statement 2	NULL		bind	NULL				Ebp1	NULL	full-length			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_8_2168_s_197	12682367	A GST-Ebp1 fusion protein encoding amino acids 293 - 372 (encompassing the HDAC2 binding domain) bound HDAC enzymatic activity as well as full-length Ebp1.	bind
45379	5	10488	7	NULL	NULL	0	NULL	GST-Ebp1 	NULL		is a type of	NULL				fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_8_2168_s_197	12682367	A GST-Ebp1 fusion protein encoding amino acids 293 - 372 (encompassing the HDAC2 binding domain) bound HDAC enzymatic activity as well as full-length Ebp1.	bind
39114	1	10489	6	13	NULL	NULL	NULL	GST-fusion protein	GP		contains					l-afadin	GP		PDZ domain		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_3_539_s_153	10225955	A GST-fusion protein  of the PDZ domain of l-afadin (GST-l-afadin-PDZ)  bound to a Myc-tagged protein of the cytoplasmic region  of nectin-1 (Myc-nectin-1-CP) immobilized on protein  A-Sepharose beads through the anti-Myc mAb (Fig.  2 A).	bind
39115	2	10489	6	13	NULL	NULL	NULL	statement 1	GP		is					GST-1-afadin-PDZ	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_3_539_s_153	10225955	A GST-fusion protein  of the PDZ domain of l-afadin (GST-l-afadin-PDZ)  bound to a Myc-tagged protein of the cytoplasmic region  of nectin-1 (Myc-nectin-1-CP) immobilized on protein  A-Sepharose beads through the anti-Myc mAb (Fig.  2 A).	bind
39116	3	10489	6	13	NULL	NULL	NULL	nectin-1	GP	Myc-tagged	is			cytoplasmic region		Myc-nectin-1-CP	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_3_539_s_153	10225955	A GST-fusion protein  of the PDZ domain of l-afadin (GST-l-afadin-PDZ)  bound to a Myc-tagged protein of the cytoplasmic region  of nectin-1 (Myc-nectin-1-CP) immobilized on protein  A-Sepharose beads through the anti-Myc mAb (Fig.  2 A).	bind
39117	4	10489	6	13	NULL	NULL	NULL	GST-l-afadin-PDZ	GP		bind					Myc-nectin-1-CP	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_3_539_s_153	10225955	A GST-fusion protein  of the PDZ domain of l-afadin (GST-l-afadin-PDZ)  bound to a Myc-tagged protein of the cytoplasmic region  of nectin-1 (Myc-nectin-1-CP) immobilized on protein  A-Sepharose beads through the anti-Myc mAb (Fig.  2 A).	bind
45380	1	10489	7	NULL	NULL	0	NULL	GST-l-afadin-PDZ	NULL		bind	NULL				Myc-nectin-1-CP	NULL	immobilized			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_3_539_s_153	10225955	A GST-fusion protein  of the PDZ domain of l-afadin (GST-l-afadin-PDZ)  bound to a Myc-tagged protein of the cytoplasmic region  of nectin-1 (Myc-nectin-1-CP) immobilized on protein  A-Sepharose beads through the anti-Myc mAb (Fig.  2 A).	bind
45381	2	10489	7	NULL	NULL	0	NULL	GST-l-afadin-PDZ	NULL		is	NULL				l-afadin 	NULL		PDZ domain		NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_3_539_s_153	10225955	A GST-fusion protein  of the PDZ domain of l-afadin (GST-l-afadin-PDZ)  bound to a Myc-tagged protein of the cytoplasmic region  of nectin-1 (Myc-nectin-1-CP) immobilized on protein  A-Sepharose beads through the anti-Myc mAb (Fig.  2 A).	bind
45382	3	10489	7	NULL	NULL	0	NULL	statement 2	NULL		is a type of	NULL				GST-fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_3_539_s_153	10225955	A GST-fusion protein  of the PDZ domain of l-afadin (GST-l-afadin-PDZ)  bound to a Myc-tagged protein of the cytoplasmic region  of nectin-1 (Myc-nectin-1-CP) immobilized on protein  A-Sepharose beads through the anti-Myc mAb (Fig.  2 A).	bind
45383	4	10489	7	NULL	NULL	0	NULL	Myc-nectin-1-CP	NULL		is	NULL				nectin-1	NULL		cytoplasmic region of		NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_3_539_s_153	10225955	A GST-fusion protein  of the PDZ domain of l-afadin (GST-l-afadin-PDZ)  bound to a Myc-tagged protein of the cytoplasmic region  of nectin-1 (Myc-nectin-1-CP) immobilized on protein  A-Sepharose beads through the anti-Myc mAb (Fig.  2 A).	bind
45384	5	10489	7	NULL	NULL	0	NULL	statement 4	NULL		is a type of	NULL				Myc-tagged protein 	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_3_539_s_153	10225955	A GST-fusion protein  of the PDZ domain of l-afadin (GST-l-afadin-PDZ)  bound to a Myc-tagged protein of the cytoplasmic region  of nectin-1 (Myc-nectin-1-CP) immobilized on protein  A-Sepharose beads through the anti-Myc mAb (Fig.  2 A).	bind
38934	1	10490	6	13	NULL	NULL	NULL	GST-fusion protein	GP		carry					hSet2/HYPB	GP		residues 1,884 - 2,061		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_49_17636_s_30	16314571	A GST-fusion protein carrying residues 1,884 - 2,061 of hSet2/HYPB, containing a WW domain and a putative SRI domain, was expressed in and purified from bacterial cells (see  Supporting Text, which is published as  supporting information on the PNAS web site, for detailed procedures); far-Western blotting (performed as described in ref.  ) confirmed that this fusion protein binds the PCTD.	bind
38935	2	10490	6	13	NULL	NULL	NULL	GST-fusion protein	GP		contains								WW domain		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_49_17636_s_30	16314571	A GST-fusion protein carrying residues 1,884 - 2,061 of hSet2/HYPB, containing a WW domain and a putative SRI domain, was expressed in and purified from bacterial cells (see  Supporting Text, which is published as  supporting information on the PNAS web site, for detailed procedures); far-Western blotting (performed as described in ref.  ) confirmed that this fusion protein binds the PCTD.	bind
38936	3	10490	6	13	NULL	NULL	NULL	GST-fusion protein	GP		contains							putative	SRI domain		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_49_17636_s_30	16314571	A GST-fusion protein carrying residues 1,884 - 2,061 of hSet2/HYPB, containing a WW domain and a putative SRI domain, was expressed in and purified from bacterial cells (see  Supporting Text, which is published as  supporting information on the PNAS web site, for detailed procedures); far-Western blotting (performed as described in ref.  ) confirmed that this fusion protein binds the PCTD.	bind
38937	4	10490	6	13	NULL	NULL	NULL	GST-fusion protein	GP		bind					PCTD	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_49_17636_s_30	16314571	A GST-fusion protein carrying residues 1,884 - 2,061 of hSet2/HYPB, containing a WW domain and a putative SRI domain, was expressed in and purified from bacterial cells (see  Supporting Text, which is published as  supporting information on the PNAS web site, for detailed procedures); far-Western blotting (performed as described in ref.  ) confirmed that this fusion protein binds the PCTD.	bind
45385	1	10490	7	NULL	NULL	0	NULL	GST-fusion protein	NULL		contains	NULL				hSet2/HYPB	NULL		residues 1,884 - 2,061		NULL		0	NULL	NULL	NULL	gw70_pnas_102_49_17636_s_30	16314571	A GST-fusion protein carrying residues 1,884 - 2,061 of hSet2/HYPB, containing a WW domain and a putative SRI domain, was expressed in and purified from bacterial cells (see  Supporting Text, which is published as  supporting information on the PNAS web site, for detailed procedures); far-Western blotting (performed as described in ref.  ) confirmed that this fusion protein binds the PCTD.	bind
45572	2	10490	7	10	NULL	0	NULL	GST-fusion protein			contains								WW domain		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_49_17636_s_30	16314571	A GST-fusion protein carrying residues 1,884 - 2,061 of hSet2/HYPB, containing a WW domain and a putative SRI domain, was expressed in and purified from bacterial cells (see  Supporting Text, which is published as  supporting information on the PNAS web site, for detailed procedures); far-Western blotting (performed as described in ref.  ) confirmed that this fusion protein binds the PCTD.	bind
45573	3	10490	7	10	NULL	0	NULL	GST-fusion protein			contains							putative	SRI domain		NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_49_17636_s_30	16314571	A GST-fusion protein carrying residues 1,884 - 2,061 of hSet2/HYPB, containing a WW domain and a putative SRI domain, was expressed in and purified from bacterial cells (see  Supporting Text, which is published as  supporting information on the PNAS web site, for detailed procedures); far-Western blotting (performed as described in ref.  ) confirmed that this fusion protein binds the PCTD.	bind
45575	5	10490	7	NULL	NULL	0	NULL	statement 1	NULL		occur along  with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_49_17636_s_30	16314571	A GST-fusion protein carrying residues 1,884 - 2,061 of hSet2/HYPB, containing a WW domain and a putative SRI domain, was expressed in and purified from bacterial cells (see  Supporting Text, which is published as  supporting information on the PNAS web site, for detailed procedures); far-Western blotting (performed as described in ref.  ) confirmed that this fusion protein binds the PCTD.	bind
45576	6	10490	7	NULL	NULL	0	NULL	statement 1	NULL		occur along with	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_49_17636_s_30	16314571	A GST-fusion protein carrying residues 1,884 - 2,061 of hSet2/HYPB, containing a WW domain and a putative SRI domain, was expressed in and purified from bacterial cells (see  Supporting Text, which is published as  supporting information on the PNAS web site, for detailed procedures); far-Western blotting (performed as described in ref.  ) confirmed that this fusion protein binds the PCTD.	bind
45577	7	10490	7	NULL	NULL	0	NULL	GST-fusion protein	NULL		bind	NULL				PCTD	NULL				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_49_17636_s_30	16314571	A GST-fusion protein carrying residues 1,884 - 2,061 of hSet2/HYPB, containing a WW domain and a putative SRI domain, was expressed in and purified from bacterial cells (see  Supporting Text, which is published as  supporting information on the PNAS web site, for detailed procedures); far-Western blotting (performed as described in ref.  ) confirmed that this fusion protein binds the PCTD.	bind
38939	1	10492	6	13	NULL	NULL	NULL	GST-Fyn SH2	GP		bind		directly			Syk	GP				NULL	Jurkat-TAg cells transfected with H902-tagged Syk	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8867_s_219	9535867	A GST-Fyn SH2 fusion protein directly bound to Syk as demonstrated by Far-Western blotting of cell lysates from Jurkat-TAg cells transfected with H902-tagged Syk or with an empty vector (pME18S) (Fig.  8 A,  top panel).	bind
50222	2	10492	6	13	NULL	NULL	NULL	GST-Fyn SH2	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8867_s_219	9535867	A GST-Fyn SH2 fusion protein directly bound to Syk as demonstrated by Far-Western blotting of cell lysates from Jurkat-TAg cells transfected with H902-tagged Syk or with an empty vector (pME18S) (Fig.  8 A,  top panel).	bind
45585	1	10492	7	10	NULL	0	NULL	GST-Fyn SH2	NULL		bind	NULL	directly			Syk	NULL				NULL	Jurkat-TAg cell lysates transfected with H902-tagged Syk	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8867_s_219	9535867	A GST-Fyn SH2 fusion protein directly bound to Syk as demonstrated by Far-Western blotting of cell lysates from Jurkat-TAg cells transfected with H902-tagged Syk or with an empty vector (pME18S) (Fig.  8 A,  top panel).	bind
45586	2	10492	7	10	NULL	0	NULL	GST-Fyn SH2	NULL		is a type of	NULL				fusion protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_15_8867_s_219	9535867	A GST-Fyn SH2 fusion protein directly bound to Syk as demonstrated by Far-Western blotting of cell lysates from Jurkat-TAg cells transfected with H902-tagged Syk or with an empty vector (pME18S) (Fig.  8 A,  top panel).	bind
38940	1	10494	6	13	NULL	NULL	NULL	NS1 protein	GP	35S-labeled	bind					GST-Neb1 protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_1_7_991_s_57	9651582	A GST-Neb1 fusion protein was bound to glutathione agarose beads, and the ability of a 35S-labeled NS1 protein to bind to the GST-Neb1 protein was determined (  Figure 1B).	bind
45587	1	10494	7	NULL	NULL	0	NULL	NS1 protein	NULL	35S-labeled 	bind	NULL				GST-Neb1 protein	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_1_7_991_s_57	9651582	A GST-Neb1 fusion protein was bound to glutathione agarose beads, and the ability of a 35S-labeled NS1 protein to bind to the GST-Neb1 protein was determined (  Figure 1B).	bind
38941	1	10495	6	13	NULL	NULL	NULL	GST-PFD	GP		bind		specifically			gD260t	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_26_9323_s_241	15972328	A GST-PFD fusion protein specifically bound gD260t or longer forms of gD.	bind
38942	2	10495	6	13	NULL	NULL	NULL	GST-PFD	GP		bind		specifically			gD	GP	longer forms of 			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_26_9323_s_241	15972328	A GST-PFD fusion protein specifically bound gD260t or longer forms of gD.	bind
50223	3	10495	6	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_26_9323_s_241	15972328	A GST-PFD fusion protein specifically bound gD260t or longer forms of gD.	bind
50224	4	10495	6	13	NULL	NULL	NULL	GST-PFD	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_26_9323_s_241	15972328	A GST-PFD fusion protein specifically bound gD260t or longer forms of gD.	bind
45588	1	10495	7	NULL	NULL	0	NULL	GST-PFD	NULL		bind	NULL	specifically			gD260t	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_26_9323_s_241	15972328	A GST-PFD fusion protein specifically bound gD260t or longer forms of gD.	bind
45589	2	10495	7	10	NULL	0	NULL	GST-PFD			bind		specifically			gD		longer forms of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_26_9323_s_241	15972328	A GST-PFD fusion protein specifically bound gD260t or longer forms of gD.	bind
45590	3	10495	7	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_26_9323_s_241	15972328	A GST-PFD fusion protein specifically bound gD260t or longer forms of gD.	bind
45591	4	10495	7	NULL	NULL	0	NULL	GST-PFD	NULL		is a type of	NULL				fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_26_9323_s_241	15972328	A GST-PFD fusion protein specifically bound gD260t or longer forms of gD.	bind
38943	1	10496	6	13	NULL	NULL	NULL	GST-syntenin	GP		bind					GST-syndecan-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_26_19933_s_125	10770943	A GST-syntenin fusion protein binds also to GST-syndecan-2 fusion proteins that have been fractionated by SDS-PAGE and blotted on nitrocellulose membranes ( 2).	bind
50225	2	10496	6	13	NULL	NULL	NULL	GST-syntenin	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_26_19933_s_125	10770943	A GST-syntenin fusion protein binds also to GST-syndecan-2 fusion proteins that have been fractionated by SDS-PAGE and blotted on nitrocellulose membranes ( 2).	bind
50226	3	10496	6	13	NULL	NULL	NULL	GST-syndecan-2	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_26_19933_s_125	10770943	A GST-syntenin fusion protein binds also to GST-syndecan-2 fusion proteins that have been fractionated by SDS-PAGE and blotted on nitrocellulose membranes ( 2).	bind
45592	1	10496	7	NULL	NULL	0	NULL	GST-syntenin	NULL		bind	NULL				GST-syndecan-2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_26_19933_s_125	10770943	A GST-syntenin fusion protein binds also to GST-syndecan-2 fusion proteins that have been fractionated by SDS-PAGE and blotted on nitrocellulose membranes ( 2).	bind
45593	2	10496	7	NULL	NULL	0	NULL	GST-syntenin	NULL		is a type of	NULL				fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_26_19933_s_125	10770943	A GST-syntenin fusion protein binds also to GST-syndecan-2 fusion proteins that have been fractionated by SDS-PAGE and blotted on nitrocellulose membranes ( 2).	bind
45594	3	10496	7	NULL	NULL	0	NULL	GST-syndecan-2	NULL		is a type of	NULL				fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_26_19933_s_125	10770943	A GST-syntenin fusion protein binds also to GST-syndecan-2 fusion proteins that have been fractionated by SDS-PAGE and blotted on nitrocellulose membranes ( 2).	bind
38944	1	10497	6	13	NULL	NULL	NULL	GST-TAP20	GP		bind		specifically			beta5 integrin	GP	detergent-solubilized			NULL	ECV cells	NULL	NULL	NULL	NULL	gw60_cellbiol_147_5_1073_s_251	10579726	A GST-TAP20 fusion protein coprecipitated specifically with detergent-solubilized beta5 integrin from ECV cells, and thus the binding of TAP20 to beta5 integrin does not depend on the existence of alphav.	bind
38945	2	10497	6	13	NULL	NULL	NULL	statement 1	Process		does not depend on					alphav	GP	existence of 			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_147_5_1073_s_251	10579726	A GST-TAP20 fusion protein coprecipitated specifically with detergent-solubilized beta5 integrin from ECV cells, and thus the binding of TAP20 to beta5 integrin does not depend on the existence of alphav.	bind
50227	3	10497	6	13	NULL	NULL	NULL	GST-TAP20	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_147_5_1073_s_251	10579726	A GST-TAP20 fusion protein coprecipitated specifically with detergent-solubilized beta5 integrin from ECV cells, and thus the binding of TAP20 to beta5 integrin does not depend on the existence of alphav.	bind
45595	1	10497	7	10	NULL	0	NULL	GST-TAP20			bind		specifically			beta5 integrin		detergent-solubilized			NULL	ECV cells	NULL	NULL	NULL	NULL	gw60_cellbiol_147_5_1073_s_251	10579726	A GST-TAP20 fusion protein coprecipitated specifically with detergent-solubilized beta5 integrin from ECV cells, and thus the binding of TAP20 to beta5 integrin does not depend on the existence of alphav.	bind
45596	2	10497	7	NULL	NULL	0	NULL	statement 1	NULL		does not depend on	NULL				alphav	NULL	existence of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_5_1073_s_251	10579726	A GST-TAP20 fusion protein coprecipitated specifically with detergent-solubilized beta5 integrin from ECV cells, and thus the binding of TAP20 to beta5 integrin does not depend on the existence of alphav.	bind
45597	3	10497	7	NULL	NULL	0	NULL	GST-TAP20	NULL		is a type of	NULL				fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_5_1073_s_251	10579726	A GST-TAP20 fusion protein coprecipitated specifically with detergent-solubilized beta5 integrin from ECV cells, and thus the binding of TAP20 to beta5 integrin does not depend on the existence of alphav.	bind
39118	1	10498	6	13	NULL	NULL	NULL	adenosine 3'',5''-monophosphate	Chemical	basal	regulates					surfactant protein A2 gene	GP	human			NULL	alveolar type II cells	NULL	NULL	NULL	NULL	gw70_annurevphysiol_62_0_875_s_1384	10845115	A GT box element is essential for basal and cyclic  adenosine 3'',5''-monophosphate regulation of the  human surfactant protein A2 gene in alveolar type II cells: evidence for the binding of lung nuclear proteins  distinct from Sp1.	bind
39119	3	10498	6	13	NULL	NULL	NULL				is essential for				GT box element	statement 1	Process				NULL	alveolar type II cells	NULL	NULL	NULL	NULL	gw70_annurevphysiol_62_0_875_s_1384	10845115	A GT box element is essential for basal and cyclic  adenosine 3'',5''-monophosphate regulation of the  human surfactant protein A2 gene in alveolar type II cells: evidence for the binding of lung nuclear proteins  distinct from Sp1.	bind
50762	2	10498	6	13	NULL	NULL	NULL	adenosine 3'',5''-monophosphate	Chemical	cyclic	regulates					surfactant protein A2 gene	GP	human			NULL	alveolar type II cells	NULL	NULL	NULL	NULL	gw70_annurevphysiol_62_0_875_s_1384	10845115	A GT box element is essential for basal and cyclic  adenosine 3'',5''-monophosphate regulation of the  human surfactant protein A2 gene in alveolar type II cells: evidence for the binding of lung nuclear proteins  distinct from Sp1.	bind
50763	4	10498	6	13	NULL	NULL	NULL				is essential for				GT box element	statement 2	Process				NULL	alveolar type II cells	NULL	NULL	NULL	NULL	gw70_annurevphysiol_62_0_875_s_1384	10845115	A GT box element is essential for basal and cyclic  adenosine 3'',5''-monophosphate regulation of the  human surfactant protein A2 gene in alveolar type II cells: evidence for the binding of lung nuclear proteins  distinct from Sp1.	bind
50764	5	10498	6	13	NULL	NULL	NULL	lung nuclear proteins	GP	binding of	is distinct from					Sp1	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_62_0_875_s_1384	10845115	A GT box element is essential for basal and cyclic  adenosine 3'',5''-monophosphate regulation of the  human surfactant protein A2 gene in alveolar type II cells: evidence for the binding of lung nuclear proteins  distinct from Sp1.	bind
45598	1	10498	7	NULL	NULL	0	NULL	adenosine 3'',5''-monophosphate	NULL	basal	regulates	NULL				surfactant protein A2 gene	NULL	human			NULL	 alveolar type II cells	0	NULL	NULL	NULL	gw70_annurevphysiol_62_0_875_s_1384	10845115	A GT box element is essential for basal and cyclic  adenosine 3'',5''-monophosphate regulation of the  human surfactant protein A2 gene in alveolar type II cells: evidence for the binding of lung nuclear proteins  distinct from Sp1.	bind
45599	2	10498	7	NULL	NULL	0	NULL	adenosine 3'',5''-monophosphate	NULL	cyclic	regulates	NULL				surfactant protein A2 gene	NULL	human			NULL	alveolar type II cells	0	NULL	NULL	NULL	gw70_annurevphysiol_62_0_875_s_1384	10845115	A GT box element is essential for basal and cyclic  adenosine 3'',5''-monophosphate regulation of the  human surfactant protein A2 gene in alveolar type II cells: evidence for the binding of lung nuclear proteins  distinct from Sp1.	bind
45600	3	10498	7	10	NULL	0	NULL				is essential for				GT box element	statement 1					NULL	alveolar type II cells	NULL	NULL	NULL	NULL	gw70_annurevphysiol_62_0_875_s_1384	10845115	A GT box element is essential for basal and cyclic  adenosine 3'',5''-monophosphate regulation of the  human surfactant protein A2 gene in alveolar type II cells: evidence for the binding of lung nuclear proteins  distinct from Sp1.	bind
45601	4	10498	7	10	NULL	0	NULL				is essential for				GT box element	statement 2					NULL	alveolar type II cells	NULL	NULL	NULL	NULL	gw70_annurevphysiol_62_0_875_s_1384	10845115	A GT box element is essential for basal and cyclic  adenosine 3'',5''-monophosphate regulation of the  human surfactant protein A2 gene in alveolar type II cells: evidence for the binding of lung nuclear proteins  distinct from Sp1.	bind
45602	5	10498	7	NULL	NULL	0	NULL	lung nuclear proteins	NULL	binding of	is distinct from	NULL				Sp1	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevphysiol_62_0_875_s_1384	10845115	A GT box element is essential for basal and cyclic  adenosine 3'',5''-monophosphate regulation of the  human surfactant protein A2 gene in alveolar type II cells: evidence for the binding of lung nuclear proteins  distinct from Sp1.	bind
38946	1	10502	6	13	NULL	NULL	NULL	Ran	GP	yeast	bind			G21V		GTP	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_31_0_277_s_295	9442897	A GTP-bound form of yeast Ran (G21V;  146), as well as mutations in  YRB1 ( 147), and in  RNA1 ( 25,  95), block nuclear protein import and the appearance of poly	bind
38947	2	10502	6	13	NULL	NULL	NULL	RNA1	GP	mutant	blocks					nuclear protein	GP	import of			NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_31_0_277_s_295	9442897	A GTP-bound form of yeast Ran (G21V;  146), as well as mutations in  YRB1 ( 147), and in  RNA1 ( 25,  95), block nuclear protein import and the appearance of poly	bind
38948	3	10502	6	13	NULL	NULL	NULL	YRB1	GP	mutant	blocks					nuclear protein	GP	import of			NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_31_0_277_s_295	9442897	A GTP-bound form of yeast Ran (G21V;  146), as well as mutations in  YRB1 ( 147), and in  RNA1 ( 25,  95), block nuclear protein import and the appearance of poly	bind
38949	4	10502	6	13	NULL	NULL	NULL	statement 1	Process		blocks					nuclear protein	GP	import of			NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_31_0_277_s_295	9442897	A GTP-bound form of yeast Ran (G21V;  146), as well as mutations in  YRB1 ( 147), and in  RNA1 ( 25,  95), block nuclear protein import and the appearance of poly	bind
46219	1	10502	7	10	NULL	0	NULL	GTP	NULL		bind	NULL				Ran	NULL	yeast	G21V		NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_31_0_277_s_295	9442897	A GTP-bound form of yeast Ran (G21V;  146), as well as mutations in  YRB1 ( 147), and in  RNA1 ( 25,  95), block nuclear protein import and the appearance of poly	bind
46220	2	10502	7	10	NULL	0	NULL	statement 1	NULL		block	NULL				nuclear protein	NULL	import of			NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_31_0_277_s_295	9442897	A GTP-bound form of yeast Ran (G21V;  146), as well as mutations in  YRB1 ( 147), and in  RNA1 ( 25,  95), block nuclear protein import and the appearance of poly	bind
46221	3	10502	7	10	NULL	0	NULL	YRB1	NULL	mutant	block	NULL				nuclear protein	NULL	import of			NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_31_0_277_s_295	9442897	A GTP-bound form of yeast Ran (G21V;  146), as well as mutations in  YRB1 ( 147), and in  RNA1 ( 25,  95), block nuclear protein import and the appearance of poly	bind
46222	4	10502	7	10	NULL	0	NULL	RNA1	NULL	mutant	block	NULL				nuclear protein	NULL	import of			NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_31_0_277_s_295	9442897	A GTP-bound form of yeast Ran (G21V;  146), as well as mutations in  YRB1 ( 147), and in  RNA1 ( 25,  95), block nuclear protein import and the appearance of poly	bind
38950	1	10503	6	13	NULL	NULL	NULL	GBD	GP		is					GTPase-binding domain	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_35761_s_28	11459849	A GTPase-binding domain (GBD) binds Cdc42, a Rho family GTPase ( 14).	bind
38951	2	10503	6	13	NULL	NULL	NULL				bind			GBD		Cdc42	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_35761_s_28	11459849	A GTPase-binding domain (GBD) binds Cdc42, a Rho family GTPase ( 14).	bind
38952	3	10503	6	13	NULL	NULL	NULL	Cdc42	GP		is a type of					Rho family GTPase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_35761_s_28	11459849	A GTPase-binding domain (GBD) binds Cdc42, a Rho family GTPase ( 14).	bind
46223	1	10503	7	NULL	NULL	0	NULL		NULL		binds	NULL		GBD		Cdc42	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_38_35761_s_28	11459849	A GTPase-binding domain (GBD) binds Cdc42, a Rho family GTPase ( 14).	bind
46224	2	10503	7	10	NULL	0	NULL	GBD	NULL		is	NULL				GTPase-binding domain	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_35761_s_28	11459849	A GTPase-binding domain (GBD) binds Cdc42, a Rho family GTPase ( 14).	bind
46225	3	10503	7	NULL	NULL	0	NULL	Cdc42	NULL		is a type of	NULL				Rho family GTPase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_38_35761_s_28	11459849	A GTPase-binding domain (GBD) binds Cdc42, a Rho family GTPase ( 14).	bind
38953	1	10504	6	13	NULL	NULL	NULL	guanine nucleotide exchange factor for Ras	GP		bind					GRB2	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_18_2295_s_824	9308960	A guanine nucleotide exchange factor for Ras that binds to GRB2.	bind
46227	1	10504	7	10	NULL	0	NULL	guanine nucleotide exchange factor for Ras	NULL		bind	NULL				GRB2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_18_2295_s_824	9308960	A guanine nucleotide exchange factor for Ras that binds to GRB2.	bind
38954	1	10506	6	13	NULL	NULL	NULL	UNC-18	GP		bind					Ce syntaxin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_19_12_4772_s_93	10366611	A half-maximal binding (ED50) of UNC-18 to  Ce syntaxin occurred at 0.08 muM.	bind
46228	1	10506	7	NULL	NULL	0	NULL	UNC-18 	NULL		bind	NULL				Ce syntaxin	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_12_4772_s_93	10366611	A half-maximal binding (ED50) of UNC-18 to  Ce syntaxin occurred at 0.08 muM.	bind
38955	1	10507	6	13	NULL	NULL	NULL	dopamine	Chemical		bind					NCS	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_37_33878_s_136	12107162	A Hanes plot ([substrate concentration] nH V 1 versus [substrate concentration] nH), where  nH = 1.8, also produced a linear function confirming the positive cooperativity of dopamine binding to NCS at a saturating level of 4-HPAA. Varying the concentration of 4-HPAA from 0.2 to 1.3 mM at a saturating level (280 muM) of dopamine produced hyperbolic saturation kinetics, indicating the lack of cooperativity in the binding of 4-HPAA to purified NCS.	bind
38956	2	10507	6	13	NULL	NULL	NULL	4-HPAA	GP		bind					NCS	GP	purified			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_37_33878_s_136	12107162	A Hanes plot ([substrate concentration] nH V 1 versus [substrate concentration] nH), where  nH = 1.8, also produced a linear function confirming the positive cooperativity of dopamine binding to NCS at a saturating level of 4-HPAA. Varying the concentration of 4-HPAA from 0.2 to 1.3 mM at a saturating level (280 muM) of dopamine produced hyperbolic saturation kinetics, indicating the lack of cooperativity in the binding of 4-HPAA to purified NCS.	bind
46229	1	10507	7	NULL	NULL	0	NULL	dopamine	NULL		bind	NULL				NCS	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_37_33878_s_136	12107162	A Hanes plot ([substrate concentration] nH V 1 versus [substrate concentration] nH), where  nH = 1.8, also produced a linear function confirming the positive cooperativity of dopamine binding to NCS at a saturating level of 4-HPAA. Varying the concentration of 4-HPAA from 0.2 to 1.3 mM at a saturating level (280 muM) of dopamine produced hyperbolic saturation kinetics, indicating the lack of cooperativity in the binding of 4-HPAA to purified NCS.	bind
46230	2	10507	7	NULL	NULL	0	NULL	 4-HPAA	NULL		bind	NULL				NCS	NULL	purified			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_37_33878_s_136	12107162	A Hanes plot ([substrate concentration] nH V 1 versus [substrate concentration] nH), where  nH = 1.8, also produced a linear function confirming the positive cooperativity of dopamine binding to NCS at a saturating level of 4-HPAA. Varying the concentration of 4-HPAA from 0.2 to 1.3 mM at a saturating level (280 muM) of dopamine produced hyperbolic saturation kinetics, indicating the lack of cooperativity in the binding of 4-HPAA to purified NCS.	bind
39120	1	10508	6	13	NULL	NULL	NULL	PRT1 - TIF34 - TIF35 subcomplex	GP		does not bind					TIF32-delta5-His	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_21_5886_s_198	12411506	A hc plasmid with  PRT1,  TIF34 and  TIF35 did not suppress the Slg -  phenotype of hc  TIF32-delta5-His (Figure  5D, sector 3 versus 5), in agreement with the fact that the PRT1 - TIF34 - TIF35 subcomplex does not bind to TIF32-delta5-His.	bind
46231	1	10508	7	NULL	NULL	0	NULL	PRT1 - TIF34 - TIF35 subcomplex	NULL		does not bind	NULL				TIF32-delta5-His	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_21_21_5886_s_198	12411506	A hc plasmid with  PRT1,  TIF34 and  TIF35 did not suppress the Slg -  phenotype of hc  TIF32-delta5-His (Figure  5D, sector 3 versus 5), in agreement with the fact that the PRT1 - TIF34 - TIF35 subcomplex does not bind to TIF32-delta5-His.	bind
38958	1	10509	6	13	NULL	NULL	NULL	head-to-tail monomer of Fu	GP		bind					Cos2	Cell				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_23_10397_s_86	15542847	A head-to-tail monomer of Fu binds Cos2.	bind
46232	1	10509	7	10	NULL	0	NULL	 head-to-tail monomer of Fu	NULL		bind	NULL				Cos2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_23_10397_s_86	15542847	A head-to-tail monomer of Fu binds Cos2.	bind
38959	1	10510	6	13	NULL	NULL	NULL	HSF1	GP	human	regulates			heat shock-responsive domain				function of	transcription activation domain		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_4949_s_450	9710578	A heat shock-responsive domain of human HSF1 that regulates transcription activation domain function.	bind
46233	1	10510	7	NULL	NULL	0	NULL	 HSF1	NULL	human	regulates	NULL		heat shock-responsive domain			NULL	function of	transcription activation domain		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_9_4949_s_450	9710578	A heat shock-responsive domain of human HSF1 that regulates transcription activation domain function.	bind
50815	1	10512	6	13	NULL	NULL	NULL	helicase	GP		catalyse					43 nucleotide DNA fragment	NucleicAcid	displacement of 			NULL		NULL	NULL	NULL	NULL	gw70_yeast_22_16_1269_s_255	16358299	A helicase that binds and translocates 5   3  will catalyse displacement of the 43 nucleotide DNA fragment.	bind
46234	1	10512	7	NULL	NULL	0	NULL	helicase	NULL		catalyse	NULL				43 nucleotide DNA fragment	NULL	displacement of			NULL		0	NULL	NULL	NULL	gw70_yeast_22_16_1269_s_255	16358299	A helicase that binds and translocates 5   3  will catalyse displacement of the 43 nucleotide DNA fragment.	bind
38962	1	10513	6	13	NULL	NULL	NULL	helix-loop-helix zipper protein	GP		forms a complex with		sequence specifically			Myc	GP				NULL		NULL	NULL	NULL	NULL	gw60_gene_216_1_155_s_181	9714786	A helix-loop-helix zipper protein that forms a sequence specific DNA binding complex with Myc.	bind
46235	1	10513	7	10	NULL	0	NULL	helix-loop-helix zipper protein	NULL		forms complex with	NULL	sequence specifically			Myc 	NULL				NULL		NULL	NULL	NULL	NULL	gw60_gene_216_1_155_s_181	9714786	A helix-loop-helix zipper protein that forms a sequence specific DNA binding complex with Myc.	bind
38964	1	10514	6	13	NULL	NULL	NULL	basic fibroblast growth factor	GP		is a type of					angiogenic protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_82_3_321_s_307	9486660	A heparin binding angiogenic protein -- basic fibroblast growth factor -- is stored within basement membrane.	bind
38965	2	10514	6	13	NULL	NULL	NULL	basic fibroblast growth factor	GP		bind					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_82_3_321_s_307	9486660	A heparin binding angiogenic protein -- basic fibroblast growth factor -- is stored within basement membrane.	bind
38966	3	10514	6	13	NULL	NULL	NULL	basic fibroblast growth factor	GP		is stored within					basement membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_82_3_321_s_307	9486660	A heparin binding angiogenic protein -- basic fibroblast growth factor -- is stored within basement membrane.	bind
46237	1	10514	7	10	NULL	0	NULL	basic fibroblast growth factor	NULL		is a type of	NULL				angiogenic protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_82_3_321_s_307	9486660	A heparin binding angiogenic protein -- basic fibroblast growth factor -- is stored within basement membrane.	bind
46238	2	10514	7	NULL	NULL	0	NULL	basic fibroblast growth factor	NULL		is stored within	NULL				basement membrane	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_82_3_321_s_307	9486660	A heparin binding angiogenic protein -- basic fibroblast growth factor -- is stored within basement membrane.	bind
50230	3	10514	7	10	NULL	0	NULL	\tbasic fibroblast growth factor	NULL		bind	NULL				heparin	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_82_3_321_s_307	9486660	A heparin binding angiogenic protein -- basic fibroblast growth factor -- is stored within basement membrane.	bind
38967	1	10515	6	13	NULL	NULL	NULL	heparin	Chemical		bind					gp120	GP		V3 loop		NULL		NULL	NULL	NULL	NULL	gw70_neuroscience_128_1_143_s_285	15450361	A heparin site on gp120 for initial binding  is consistent with work showing that heparin binds to the V3 loop of gp120 to block  HIV-1 infectivity (  Harrop and Rider, 1998;   Rider, 1997).	bind
38969	2	10515	6	13	NULL	NULL	NULL	statement 1	Process		block					HIV-1	Organism	infectivity of			NULL		NULL	NULL	NULL	NULL	gw70_neuroscience_128_1_143_s_285	15450361	A heparin site on gp120 for initial binding  is consistent with work showing that heparin binds to the V3 loop of gp120 to block  HIV-1 infectivity (  Harrop and Rider, 1998;   Rider, 1997).	bind
46239	1	10515	7	NULL	NULL	0	NULL	heparin	NULL		bind	NULL				gp120	NULL		V3 loop		NULL		0	NULL	NULL	NULL	gw70_neuroscience_128_1_143_s_285	15450361	A heparin site on gp120 for initial binding  is consistent with work showing that heparin binds to the V3 loop of gp120 to block  HIV-1 infectivity (  Harrop and Rider, 1998;   Rider, 1997).	bind
46240	2	10515	7	10	NULL	0	NULL	statement 1			block					HIV-1		infectivity of			NULL		NULL	NULL	NULL	NULL	gw70_neuroscience_128_1_143_s_285	15450361	A heparin site on gp120 for initial binding  is consistent with work showing that heparin binds to the V3 loop of gp120 to block  HIV-1 infectivity (  Harrop and Rider, 1998;   Rider, 1997).	bind
39124	1	10516	6	13	NULL	NULL	NULL	Cyr61	GP	mutant	does not bind					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24953_s_9	10821835	A heparin-binding defective mutant of Cyr61 was unable to mediate fibroblast adhesion through integrin alpha6beta1 but still mediated endothelial cell adhesion through integrin alphaVbeta3, indicating that endothelial cell adhesion through integrin alphaVbeta3 is independent of the heparin-binding activity of Cyr61.	bind
39125	2	10516	6	13	NULL	NULL	NULL	statement 1	Process		does not mediate					fibroblast	Cell	adhesion of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24953_s_9	10821835	A heparin-binding defective mutant of Cyr61 was unable to mediate fibroblast adhesion through integrin alpha6beta1 but still mediated endothelial cell adhesion through integrin alphaVbeta3, indicating that endothelial cell adhesion through integrin alphaVbeta3 is independent of the heparin-binding activity of Cyr61.	bind
39126	3	10516	6	13	NULL	NULL	NULL	statement 2	Process		occurs through					integrin alpha6beta1 	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24953_s_9	10821835	A heparin-binding defective mutant of Cyr61 was unable to mediate fibroblast adhesion through integrin alpha6beta1 but still mediated endothelial cell adhesion through integrin alphaVbeta3, indicating that endothelial cell adhesion through integrin alphaVbeta3 is independent of the heparin-binding activity of Cyr61.	bind
39127	4	10516	6	13	NULL	NULL	NULL	statement 1	Process		mediates					endothelial cells	Cell	adhesion of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24953_s_9	10821835	A heparin-binding defective mutant of Cyr61 was unable to mediate fibroblast adhesion through integrin alpha6beta1 but still mediated endothelial cell adhesion through integrin alphaVbeta3, indicating that endothelial cell adhesion through integrin alphaVbeta3 is independent of the heparin-binding activity of Cyr61.	bind
39128	5	10516	6	13	NULL	NULL	NULL	statement 4	Process		occurs through					integrin alphaVbeta3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24953_s_9	10821835	A heparin-binding defective mutant of Cyr61 was unable to mediate fibroblast adhesion through integrin alpha6beta1 but still mediated endothelial cell adhesion through integrin alphaVbeta3, indicating that endothelial cell adhesion through integrin alphaVbeta3 is independent of the heparin-binding activity of Cyr61.	bind
39129	6	10516	6	13	NULL	NULL	NULL	statement 5	Process		is independent of					Cyr61	GP	heparin-binding activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24953_s_9	10821835	A heparin-binding defective mutant of Cyr61 was unable to mediate fibroblast adhesion through integrin alpha6beta1 but still mediated endothelial cell adhesion through integrin alphaVbeta3, indicating that endothelial cell adhesion through integrin alphaVbeta3 is independent of the heparin-binding activity of Cyr61.	bind
48699	1	10516	7	NULL	NULL	0	NULL	fibroblast	NULL	adhesion of	occur through	NULL				integrin alpha6beta1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24953_s_9	10821835	A heparin-binding defective mutant of Cyr61 was unable to mediate fibroblast adhesion through integrin alpha6beta1 but still mediated endothelial cell adhesion through integrin alphaVbeta3, indicating that endothelial cell adhesion through integrin alphaVbeta3 is independent of the heparin-binding activity of Cyr61.	bind
48700	2	10516	7	10	NULL	0	NULL	statement 6	NULL		does not mediate	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24953_s_9	10821835	A heparin-binding defective mutant of Cyr61 was unable to mediate fibroblast adhesion through integrin alpha6beta1 but still mediated endothelial cell adhesion through integrin alphaVbeta3, indicating that endothelial cell adhesion through integrin alphaVbeta3 is independent of the heparin-binding activity of Cyr61.	bind
48701	3	10516	7	NULL	NULL	0	NULL	endothelial cell	NULL	adhesion of	occur through	NULL				integrin alphaVbeta3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24953_s_9	10821835	A heparin-binding defective mutant of Cyr61 was unable to mediate fibroblast adhesion through integrin alpha6beta1 but still mediated endothelial cell adhesion through integrin alphaVbeta3, indicating that endothelial cell adhesion through integrin alphaVbeta3 is independent of the heparin-binding activity of Cyr61.	bind
48702	4	10516	7	10	NULL	0	NULL	statement 6	NULL		mediate	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24953_s_9	10821835	A heparin-binding defective mutant of Cyr61 was unable to mediate fibroblast adhesion through integrin alpha6beta1 but still mediated endothelial cell adhesion through integrin alphaVbeta3, indicating that endothelial cell adhesion through integrin alphaVbeta3 is independent of the heparin-binding activity of Cyr61.	bind
48703	5	10516	7	NULL	NULL	0	NULL	statement 4	NULL		is independent of	NULL				Cyr61	NULL	heparin-binding activity of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24953_s_9	10821835	A heparin-binding defective mutant of Cyr61 was unable to mediate fibroblast adhesion through integrin alpha6beta1 but still mediated endothelial cell adhesion through integrin alphaVbeta3, indicating that endothelial cell adhesion through integrin alphaVbeta3 is independent of the heparin-binding activity of Cyr61.	bind
50231	6	10516	7	10	NULL	0	NULL	Cyr61	NULL	mutant	does not bind	NULL				heparin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24953_s_9	10821835	A heparin-binding defective mutant of Cyr61 was unable to mediate fibroblast adhesion through integrin alpha6beta1 but still mediated endothelial cell adhesion through integrin alphaVbeta3, indicating that endothelial cell adhesion through integrin alphaVbeta3 is independent of the heparin-binding activity of Cyr61.	bind
38974	1	10517	6	13	NULL	NULL	NULL	HEPES molecule	GP		bind							putative	K domain in the lysine-binding pocket		NULL		NULL	NULL	NULL	NULL	gw60_embo_20_20_5543_s_37	11597998	A HEPES molecule is bound to each of the K domains in the putative lysine-binding pocket, as in the 1bht structure ( Ultsch  et al., 1998).	bind
48704	1	10517	7	10	NULL	0	NULL	HEPES molecule	NULL		bind	NULL					NULL	putative	K domains in lysine-binding pocket		NULL		NULL	NULL	NULL	NULL	gw60_embo_20_20_5543_s_37	11597998	A HEPES molecule is bound to each of the K domains in the putative lysine-binding pocket, as in the 1bht structure ( Ultsch  et al., 1998).	bind
38975	1	10518	6	13	NULL	NULL	NULL	MRP8 (S100A8)	GP		forms heterocomplex with					MRP14 (S100A9)	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_6_3692_s_321	11349032	A heterocomplex formed by the calcium-binding proteins MRP8 (S100A8) and MRP14 (S100A9) binds unsaturated fatty acids with high affinity.	bind
38976	2	10518	6	13	NULL	NULL	NULL	statement 1	GP		bind		high affinity			fatty acids	Chemical	unsaturated			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_6_3692_s_321	11349032	A heterocomplex formed by the calcium-binding proteins MRP8 (S100A8) and MRP14 (S100A9) binds unsaturated fatty acids with high affinity.	bind
38977	3	10518	6	13	NULL	NULL	NULL	MRP8	GP		is a type of					calcium binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_6_3692_s_321	11349032	A heterocomplex formed by the calcium-binding proteins MRP8 (S100A8) and MRP14 (S100A9) binds unsaturated fatty acids with high affinity.	bind
38978	4	10518	6	13	NULL	NULL	NULL	MRP14	GP		is a type of					calcium binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_6_3692_s_321	11349032	A heterocomplex formed by the calcium-binding proteins MRP8 (S100A8) and MRP14 (S100A9) binds unsaturated fatty acids with high affinity.	bind
48731	1	10518	7	10	NULL	0	NULL	 MRP8(S100A8)			forms heterocomplex with					MRP14(S100A9)					NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_6_3692_s_321	11349032	A heterocomplex formed by the calcium-binding proteins MRP8 (S100A8) and MRP14 (S100A9) binds unsaturated fatty acids with high affinity.	bind
48733	2	10518	7	10	NULL	0	NULL	statement 1			bind		high affinity			 fatty acids		unsaturated			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_6_3692_s_321	11349032	A heterocomplex formed by the calcium-binding proteins MRP8 (S100A8) and MRP14 (S100A9) binds unsaturated fatty acids with high affinity.	bind
48735	3	10518	7	10	NULL	0	NULL	MRP8			is a type of					calcium binding protein					NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_6_3692_s_321	11349032	A heterocomplex formed by the calcium-binding proteins MRP8 (S100A8) and MRP14 (S100A9) binds unsaturated fatty acids with high affinity.	bind
48736	4	10518	7	10	NULL	0	NULL	 MRP14 			is a type of					calcium binding protein					NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_6_3692_s_321	11349032	A heterocomplex formed by the calcium-binding proteins MRP8 (S100A8) and MRP14 (S100A9) binds unsaturated fatty acids with high affinity.	bind
38979	1	10519	6	13	NULL	NULL	NULL	p50 subunit	GP		forms heterodimer with					p65 subunit	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_7_2927_s_17	9096323	A heterodimer composed of a p50 subunit bound to a p65 (Rel A) subunit is the common dimer.	bind
38980	2	10519	6	13	NULL	NULL	NULL	p65	GP		is					Rel A	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_7_2927_s_17	9096323	A heterodimer composed of a p50 subunit bound to a p65 (Rel A) subunit is the common dimer.	bind
48737	1	10519	7	10	NULL	0	NULL	p50 subunit 	NULL		forms heterodimer with	NULL				p65 subunit	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_7_2927_s_17	9096323	A heterodimer composed of a p50 subunit bound to a p65 (Rel A) subunit is the common dimer.	bind
48739	2	10519	7	10	NULL	0	NULL	p65 subunit	NULL		is	NULL				RelA subunit	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_7_2927_s_17	9096323	A heterodimer composed of a p50 subunit bound to a p65 (Rel A) subunit is the common dimer.	bind
38981	1	10520	6	13	NULL	NULL	NULL	STE12	GP		forms heterodimer with					TEC1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_23_7008_s_19	9384580	A heterodimer composed of STE12 and TEC1 binds to a filamentation response element (FRE), which may regulate expression of genes necessary for pseudohyphal differentiation (Laloux  et al., 1994  ; Mosch  et al., 1996  ; Madhani and Fink, 1997  ).	bind
38982	2	10520	6	13	NULL	NULL	NULL	statement 1	GP		bind									FRE	NULL		NULL	NULL	NULL	NULL	gw60_embo_16_23_7008_s_19	9384580	A heterodimer composed of STE12 and TEC1 binds to a filamentation response element (FRE), which may regulate expression of genes necessary for pseudohyphal differentiation (Laloux  et al., 1994  ; Mosch  et al., 1996  ; Madhani and Fink, 1997  ).	bind
38983	3	10520	6	13	NULL	NULL	NULL	FRE	NucleicAcid		is					filamentation response element	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_23_7008_s_19	9384580	A heterodimer composed of STE12 and TEC1 binds to a filamentation response element (FRE), which may regulate expression of genes necessary for pseudohyphal differentiation (Laloux  et al., 1994  ; Mosch  et al., 1996  ; Madhani and Fink, 1997  ).	bind
38985	4	10520	6	13	NULL	NULL	NULL	statement 2	Process		regulates		may			pseudohyphal differentiation genes	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_embo_16_23_7008_s_19	9384580	A heterodimer composed of STE12 and TEC1 binds to a filamentation response element (FRE), which may regulate expression of genes necessary for pseudohyphal differentiation (Laloux  et al., 1994  ; Mosch  et al., 1996  ; Madhani and Fink, 1997  ).	bind
48740	1	10520	7	NULL	NULL	0	NULL	STE12 	NULL		heterodimerizes with	NULL				TEC1	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_16_23_7008_s_19	9384580	A heterodimer composed of STE12 and TEC1 binds to a filamentation response element (FRE), which may regulate expression of genes necessary for pseudohyphal differentiation (Laloux  et al., 1994  ; Mosch  et al., 1996  ; Madhani and Fink, 1997  ).	bind
48741	2	10520	7	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL					NULL			FRE	NULL		0	NULL	NULL	NULL	gw60_embo_16_23_7008_s_19	9384580	A heterodimer composed of STE12 and TEC1 binds to a filamentation response element (FRE), which may regulate expression of genes necessary for pseudohyphal differentiation (Laloux  et al., 1994  ; Mosch  et al., 1996  ; Madhani and Fink, 1997  ).	bind
48742	3	10520	7	10	NULL	0	NULL	statement 2			regulate		may			pseudohyphal differentiation genes		expression of			NULL		NULL	NULL	NULL	NULL	gw60_embo_16_23_7008_s_19	9384580	A heterodimer composed of STE12 and TEC1 binds to a filamentation response element (FRE), which may regulate expression of genes necessary for pseudohyphal differentiation (Laloux  et al., 1994  ; Mosch  et al., 1996  ; Madhani and Fink, 1997  ).	bind
48743	4	10520	7	NULL	NULL	0	NULL	FRE	NULL		is	NULL				filamentation response element	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_16_23_7008_s_19	9384580	A heterodimer composed of STE12 and TEC1 binds to a filamentation response element (FRE), which may regulate expression of genes necessary for pseudohyphal differentiation (Laloux  et al., 1994  ; Mosch  et al., 1996  ; Madhani and Fink, 1997  ).	bind
39022	1	10521	6	13	NULL	NULL	NULL	USF-1/USF-2 heterodimer	GP		bind								HO HLH site		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jneurosci_23_3_807_s_256	12574409	A heterodimer of USF-1/USF-2 can bind the HO HLH site  in vitro (Lanigan and Russo, 1997  ).	bind
48744	1	10521	7	10	NULL	0	NULL	USF-1/USF-2 heterodimer			bind								HO HLH site		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jneurosci_23_3_807_s_256	12574409	A heterodimer of USF-1/USF-2 can bind the HO HLH site  in vitro (Lanigan and Russo, 1997  ).	bind
39023	1	10522	6	13	NULL	NULL	NULL	GlnRS	GP	E.coli	bind					tRNAGln transcript	NucleicAcid	yeast			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_23_16508_s_147	10347214	A heterologous RNA binding domain enhances binding of  E. coli GlnRS  to a transcript of yeast tRNAGln.	bind
50237	2	10522	6	13	NULL	NULL	NULL				enhances			heterologous RNA binding domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_23_16508_s_147	10347214	A heterologous RNA binding domain enhances binding of  E. coli GlnRS  to a transcript of yeast tRNAGln.	bind
48746	1	10522	7	NULL	NULL	0	NULL	GlnRS 	NULL	E.coli	bind	NULL				tRNAGln transcript	NULL	yeast			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_23_16508_s_147	10347214	A heterologous RNA binding domain enhances binding of  E. coli GlnRS  to a transcript of yeast tRNAGln.	bind
48747	2	10522	7	NULL	NULL	0	NULL		NULL		enhance	NULL		heterologous RNA binding domain		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_23_16508_s_147	10347214	A heterologous RNA binding domain enhances binding of  E. coli GlnRS  to a transcript of yeast tRNAGln.	bind
39024	1	10523	6	13	NULL	NULL	NULL	YRNYPT hexapeptide sequence	GP		is based on					CbpA	GP		R1/R2 region		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_22_15464_s_358	16597618	A hexapeptide (YRNYPT) sequence based on the R1/R2 region of CbpA was found to bind human SIgA by a similar peptide mapping approach.	bind
39025	2	10523	6	13	NULL	NULL	NULL	statement 1	GP		bind					SIgA	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_22_15464_s_358	16597618	A hexapeptide (YRNYPT) sequence based on the R1/R2 region of CbpA was found to bind human SIgA by a similar peptide mapping approach.	bind
48748	1	10523	7	NULL	NULL	0	NULL	YRNYPT hexapeptide	NULL		bind	NULL				SIgA	NULL	human			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_22_15464_s_358	16597618	A hexapeptide (YRNYPT) sequence based on the R1/R2 region of CbpA was found to bind human SIgA by a similar peptide mapping approach.	bind
48749	2	10523	7	NULL	NULL	0	NULL	YRNYPT hexapeptide	NULL		is based on	NULL				CbpA	NULL		R1/R2 region of		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_22_15464_s_358	16597618	A hexapeptide (YRNYPT) sequence based on the R1/R2 region of CbpA was found to bind human SIgA by a similar peptide mapping approach.	bind
39026	1	10524	6	13	NULL	NULL	NULL	BS-I-B4	GP		bind					endothelial cells	Cell	pig;; aortic			NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_308_1_19_s_106	12890473	A hexapeptide mimetic of Gal- 1,3-Gal was found by screening the hexapeptide library with the lectin BS-I-B4, which can block the binding of BS-I-B4 to pig aortic endothelial cells [ 7.	bind
39027	2	10524	6	13	NULL	NULL	NULL	hexapeptide mimetic of Gal- 1,3-Gal	GP		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_308_1_19_s_106	12890473	A hexapeptide mimetic of Gal- 1,3-Gal was found by screening the hexapeptide library with the lectin BS-I-B4, which can block the binding of BS-I-B4 to pig aortic endothelial cells [ 7.	bind
48750	1	10524	7	10	NULL	0	NULL	BS-I-B4	NULL		bind	NULL				endothelial cells	NULL	pig;;aortic			NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_308_1_19_s_106	12890473	A hexapeptide mimetic of Gal- 1,3-Gal was found by screening the hexapeptide library with the lectin BS-I-B4, which can block the binding of BS-I-B4 to pig aortic endothelial cells [ 7.	bind
48752	2	10524	7	10	NULL	0	NULL	hexapeptide mimetic of Gal- 1,3-Gal	NULL		block	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_308_1_19_s_106	12890473	A hexapeptide mimetic of Gal- 1,3-Gal was found by screening the hexapeptide library with the lectin BS-I-B4, which can block the binding of BS-I-B4 to pig aortic endothelial cells [ 7.	bind
39130	1	10525	6	13	NULL	NULL	NULL	hIGFBP-3 	GP		is substituted with			Arg75;;Leu77		hIGFBP-3	GP		Ala75;;Ala77		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10489_s_287	11784719	A hIGFBP-3 mutant with alanine substitutions at only two of the six positions, Arg75 and Leu77, also exhibited markedly decreased binding of both IGF-I and IGF-II.	bind
39132	2	10525	6	13	NULL	NULL	NULL	statement 1	Process		bind		decreased			IGF-I	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10489_s_287	11784719	A hIGFBP-3 mutant with alanine substitutions at only two of the six positions, Arg75 and Leu77, also exhibited markedly decreased binding of both IGF-I and IGF-II.	bind
39133	3	10525	6	13	NULL	NULL	NULL	statement 1	Process		bind		decreased			IGF-II	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10489_s_287	11784719	A hIGFBP-3 mutant with alanine substitutions at only two of the six positions, Arg75 and Leu77, also exhibited markedly decreased binding of both IGF-I and IGF-II.	bind
48753	1	10525	7	10	NULL	0	NULL	hIGFBP-3			is substituted with			 Arg75;;Leu77		hIGFBP-3			Ala75;;Ala77		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10489_s_287	11784719	A hIGFBP-3 mutant with alanine substitutions at only two of the six positions, Arg75 and Leu77, also exhibited markedly decreased binding of both IGF-I and IGF-II.	bind
48754	2	10525	7	10	NULL	0	NULL	statement 1			bind		decreased			IGF-I					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10489_s_287	11784719	A hIGFBP-3 mutant with alanine substitutions at only two of the six positions, Arg75 and Leu77, also exhibited markedly decreased binding of both IGF-I and IGF-II.	bind
48755	3	10525	7	10	NULL	0	NULL	statement 1			bind		decreased			IGF-II					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10489_s_287	11784719	A hIGFBP-3 mutant with alanine substitutions at only two of the six positions, Arg75 and Leu77, also exhibited markedly decreased binding of both IGF-I and IGF-II.	bind
39028	1	10526	6	13	NULL	NULL	NULL	bis-ANS	Chemical		bind		weakly			LPL	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_39_37183_s_152	12855707	A high  Ki value represents a weak binding of bis-ANS to LPL.	bind
48757	1	10526	7	NULL	NULL	0	NULL	bis-ANS	NULL		bind	NULL	weakly			LPL	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_39_37183_s_152	12855707	A high  Ki value represents a weak binding of bis-ANS to LPL.	bind
39029	1	10527	6	13	NULL	NULL	NULL	ATP	Chemical		bind					P2X7 receptor	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_39_37344_s_193	12869560	A high (low to submicromolar) and a low (>100 muM) affinity state for ATP binding to the human P2X7 receptor have been demonstrated ( ).	bind
48758	1	10527	7	NULL	NULL	0	NULL	ATP	NULL		bind	NULL				P2X7 receptor	NULL	human			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_39_37344_s_193	12869560	A high (low to submicromolar) and a low (>100 muM) affinity state for ATP binding to the human P2X7 receptor have been demonstrated ( ).	bind
39030	1	10528	6	13	NULL	NULL	NULL	GBS	Organism		bind					mAb S9	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_27_24740_s_37	12700231	A high affinity (IC50 = 23  muM) peptide ligand, FDTGAFDPDWPAC, competitively inhibited  binding of GBS not only to mAb S9 but also to polyclonal anti-GBS antibodies.	bind
39031	2	10528	6	13	NULL	NULL	NULL	GBS	Organism		bind					anti-GBS antibody	GP	polyclonal			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_27_24740_s_37	12700231	A high affinity (IC50 = 23  muM) peptide ligand, FDTGAFDPDWPAC, competitively inhibited  binding of GBS not only to mAb S9 but also to polyclonal anti-GBS antibodies.	bind
39032	3	10528	6	13	NULL	NULL	NULL	FDTGAFDPDWPAC	GP		inhibits		competitively			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_27_24740_s_37	12700231	A high affinity (IC50 = 23  muM) peptide ligand, FDTGAFDPDWPAC, competitively inhibited  binding of GBS not only to mAb S9 but also to polyclonal anti-GBS antibodies.	bind
39033	4	10528	6	13	NULL	NULL	NULL	FDTGAFDPDWPAC	GP		inhibits		competitively			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_27_24740_s_37	12700231	A high affinity (IC50 = 23  muM) peptide ligand, FDTGAFDPDWPAC, competitively inhibited  binding of GBS not only to mAb S9 but also to polyclonal anti-GBS antibodies.	bind
50238	5	10528	6	13	NULL	NULL	NULL	FDTGAFDPDWPAC	GP		is a type of					peptide ligand	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_27_24740_s_37	12700231	A high affinity (IC50 = 23  muM) peptide ligand, FDTGAFDPDWPAC, competitively inhibited  binding of GBS not only to mAb S9 but also to polyclonal anti-GBS antibodies.	bind
48759	1	10528	7	NULL	NULL	0	NULL	GBS	NULL		bind	NULL				mAb S9 	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_27_24740_s_37	12700231	A high affinity (IC50 = 23  muM) peptide ligand, FDTGAFDPDWPAC, competitively inhibited  binding of GBS not only to mAb S9 but also to polyclonal anti-GBS antibodies.	bind
48760	2	10528	7	NULL	NULL	0	NULL	GBS	NULL		bind	NULL				polyclonal anti-GBS antibodies	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_27_24740_s_37	12700231	A high affinity (IC50 = 23  muM) peptide ligand, FDTGAFDPDWPAC, competitively inhibited  binding of GBS not only to mAb S9 but also to polyclonal anti-GBS antibodies.	bind
48761	3	10528	7	NULL	NULL	0	NULL	FDTGAFDPDWPAC 	NULL		inhibit	NULL	competitively			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_27_24740_s_37	12700231	A high affinity (IC50 = 23  muM) peptide ligand, FDTGAFDPDWPAC, competitively inhibited  binding of GBS not only to mAb S9 but also to polyclonal anti-GBS antibodies.	bind
48762	4	10528	7	NULL	NULL	0	NULL	FDTGAFDPDWPAC 	NULL		inhibit	NULL	competitively			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_27_24740_s_37	12700231	A high affinity (IC50 = 23  muM) peptide ligand, FDTGAFDPDWPAC, competitively inhibited  binding of GBS not only to mAb S9 but also to polyclonal anti-GBS antibodies.	bind
48763	5	10528	7	NULL	NULL	0	NULL	FDTGAFDPDWPAC	NULL		is a type of	NULL				peptide ligand	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_27_24740_s_37	12700231	A high affinity (IC50 = 23  muM) peptide ligand, FDTGAFDPDWPAC, competitively inhibited  binding of GBS not only to mAb S9 but also to polyclonal anti-GBS antibodies.	bind
39034	1	10529	6	13	NULL	NULL	NULL	PKC	GP		bind		high affinity			Btk	GP		PH domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_20_13033_s_39	9148913	A high affinity binding between PKC and the Btk PH domain was demonstrated by this assay.	bind
48764	1	10529	7	NULL	NULL	0	NULL	 PKC	NULL		bind	NULL	high affinity			Btk	NULL		PH domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_20_13033_s_39	9148913	A high affinity binding between PKC and the Btk PH domain was demonstrated by this assay.	bind
39035	1	10530	6	13	NULL	NULL	NULL	ANS	Chemical		bind					BSP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_20_19480_s_166	15757902	A high affinity-binding site for ANS at or near the promiscuous H-site of hGST P1 - 1 has also been reported ( ,  ), in agreement with the competitive binding between ANS and BSP ( ).	bind
59040	1	10530	7	NULL	NULL	0	NULL	ANS			bind					BSP					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_19480_s_166	15757902	A high affinity-binding site for ANS at or near the promiscuous H-site of hGST P1 - 1 has also been reported ( ,  ), in agreement with the competitive binding between ANS and BSP ( ).	bind
39036	1	10531	6	13	NULL	NULL	NULL	LDL	GP		bind					LDL receptor	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_atherosclerosis_132_1_19_s_299	9247355	A high capacity, stable line for evaluating the binding of LDL to the human LDL receptor.	bind
48765	1	10531	7	NULL	NULL	0	NULL	LDL	NULL		bind	NULL				LDL receptor	NULL	human			NULL		0	NULL	NULL	NULL	gw60_atherosclerosis_132_1_19_s_299	9247355	A high capacity, stable line for evaluating the binding of LDL to the human LDL receptor.	bind
39136	1	10532	6	13	NULL	NULL	NULL	coumarin	Chemical		is a type of					CYP2A5/CYP2G1 substrates	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0560-0569_drug-metab-dispos_34_1_16221755_s_4	16221755	A high covalent binding of 2,6-diClPh-(14)C-MeSO(2) in olfactory  mucosa S9 fraction was observed, and the CYP2A5/CYP2G1 substrates coumarin  and dichlobenil significantly decreased the binding, whereas the CYP2E1  substrate chlorzoxazone had no effects.	bind
39137	2	10532	6	13	NULL	NULL	NULL	dichlobenil	Chemical		is a type of					CYP2A5/CYP2G1 substrates	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0560-0569_drug-metab-dispos_34_1_16221755_s_4	16221755	A high covalent binding of 2,6-diClPh-(14)C-MeSO(2) in olfactory  mucosa S9 fraction was observed, and the CYP2A5/CYP2G1 substrates coumarin  and dichlobenil significantly decreased the binding, whereas the CYP2E1  substrate chlorzoxazone had no effects.	bind
39138	3	10532	6	13	NULL	NULL	NULL	chlorzoxazone	Chemical		is a type of					CYP2E1 substrate	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0560-0569_drug-metab-dispos_34_1_16221755_s_4	16221755	A high covalent binding of 2,6-diClPh-(14)C-MeSO(2) in olfactory  mucosa S9 fraction was observed, and the CYP2A5/CYP2G1 substrates coumarin  and dichlobenil significantly decreased the binding, whereas the CYP2E1  substrate chlorzoxazone had no effects.	bind
39139	4	10532	6	13	NULL	NULL	NULL	coumarin	Chemical		decreases					2,6-diClPh-(14)C-MeSO(2)	Chemical	covalent binding of			NULL	olfactory mucosa S9 fraction	NULL	NULL	NULL	NULL	abs-batch0560-0569_drug-metab-dispos_34_1_16221755_s_4	16221755	A high covalent binding of 2,6-diClPh-(14)C-MeSO(2) in olfactory  mucosa S9 fraction was observed, and the CYP2A5/CYP2G1 substrates coumarin  and dichlobenil significantly decreased the binding, whereas the CYP2E1  substrate chlorzoxazone had no effects.	bind
39140	5	10532	6	13	NULL	NULL	NULL	dichlobenil	Chemical		decreases					2,6-diClPh-(14)C-MeSO(2)	Chemical	covalent binding of			NULL	olfactory mucosa S9 fraction	NULL	NULL	NULL	NULL	abs-batch0560-0569_drug-metab-dispos_34_1_16221755_s_4	16221755	A high covalent binding of 2,6-diClPh-(14)C-MeSO(2) in olfactory  mucosa S9 fraction was observed, and the CYP2A5/CYP2G1 substrates coumarin  and dichlobenil significantly decreased the binding, whereas the CYP2E1  substrate chlorzoxazone had no effects.	bind
39141	6	10532	6	13	NULL	NULL	NULL	chlorzoxazone	Chemical		has no effect in					2,6-diClPh-(14)C-MeSO(2)	Chemical	covalent binding of			NULL	olfactory mucosa S9 fraction	NULL	NULL	NULL	NULL	abs-batch0560-0569_drug-metab-dispos_34_1_16221755_s_4	16221755	A high covalent binding of 2,6-diClPh-(14)C-MeSO(2) in olfactory  mucosa S9 fraction was observed, and the CYP2A5/CYP2G1 substrates coumarin  and dichlobenil significantly decreased the binding, whereas the CYP2E1  substrate chlorzoxazone had no effects.	bind
48767	1	10532	7	10	NULL	0	NULL	coumarin			decrease					 2,6-diClPh-(14)C-MeSO(2)		covalent binding of			NULL	 olfactory mucosa S9 fraction	NULL	NULL	NULL	NULL	abs-batch0560-0569_drug-metab-dispos_34_1_16221755_s_4	16221755	A high covalent binding of 2,6-diClPh-(14)C-MeSO(2) in olfactory  mucosa S9 fraction was observed, and the CYP2A5/CYP2G1 substrates coumarin  and dichlobenil significantly decreased the binding, whereas the CYP2E1  substrate chlorzoxazone had no effects.	bind
48768	2	10532	7	10	NULL	0	NULL	dichlobenil 			decrease					2,6-diClPh-(14)C-MeSO(2)		covalent binding of			NULL	olfactory mucosa S9 fraction	NULL	NULL	NULL	NULL	abs-batch0560-0569_drug-metab-dispos_34_1_16221755_s_4	16221755	A high covalent binding of 2,6-diClPh-(14)C-MeSO(2) in olfactory  mucosa S9 fraction was observed, and the CYP2A5/CYP2G1 substrates coumarin  and dichlobenil significantly decreased the binding, whereas the CYP2E1  substrate chlorzoxazone had no effects.	bind
48769	3	10532	7	10	NULL	0	NULL	chlorzoxazone			does not effect					2,6-diClPh-(14)C-MeSO(2)		covalent binding of 			NULL	olfactory mucosa S9 fraction	NULL	NULL	NULL	NULL	abs-batch0560-0569_drug-metab-dispos_34_1_16221755_s_4	16221755	A high covalent binding of 2,6-diClPh-(14)C-MeSO(2) in olfactory  mucosa S9 fraction was observed, and the CYP2A5/CYP2G1 substrates coumarin  and dichlobenil significantly decreased the binding, whereas the CYP2E1  substrate chlorzoxazone had no effects.	bind
48770	5	10532	7	NULL	NULL	0	NULL	coumarin	NULL		is a type of	NULL				CYP2A5/CYP2G1 substrates	NULL				NULL		0	NULL	NULL	NULL	abs-batch0560-0569_drug-metab-dispos_34_1_16221755_s_4	16221755	A high covalent binding of 2,6-diClPh-(14)C-MeSO(2) in olfactory  mucosa S9 fraction was observed, and the CYP2A5/CYP2G1 substrates coumarin  and dichlobenil significantly decreased the binding, whereas the CYP2E1  substrate chlorzoxazone had no effects.	bind
48771	6	10532	7	NULL	NULL	0	NULL	dichlobenil	NULL		is a type of	NULL				CYP2A5/CYP2G1 substrates	NULL				NULL		0	NULL	NULL	NULL	abs-batch0560-0569_drug-metab-dispos_34_1_16221755_s_4	16221755	A high covalent binding of 2,6-diClPh-(14)C-MeSO(2) in olfactory  mucosa S9 fraction was observed, and the CYP2A5/CYP2G1 substrates coumarin  and dichlobenil significantly decreased the binding, whereas the CYP2E1  substrate chlorzoxazone had no effects.	bind
48772	4	10532	7	10	NULL	0	NULL	chlorzoxazone			is a type of					CYP2E1 substrate					NULL		NULL	NULL	NULL	NULL	abs-batch0560-0569_drug-metab-dispos_34_1_16221755_s_4	16221755	A high covalent binding of 2,6-diClPh-(14)C-MeSO(2) in olfactory  mucosa S9 fraction was observed, and the CYP2A5/CYP2G1 substrates coumarin  and dichlobenil significantly decreased the binding, whereas the CYP2E1  substrate chlorzoxazone had no effects.	bind
39037	1	10534	6	13	NULL	NULL	NULL	MURA	GP		does not bind					Mu5 transposon	NucleicAcid	inactive	divergent left TIR		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_genetics_160_2_697_s_410	11861572	A high degree of conservation in this predicted binding site is thought to be required for MURA binding because MURA fails to bind  in vitro to the divergent left TIR of the apparently inactive  Mu5 transposon ( B ENITO and WALBOT 1997   ).	bind
48787	1	10534	7	NULL	NULL	0	NULL	MURA 	NULL		does not bind	NULL				Mu5 transposon	NULL	inactive	divergent left TIR		NULL	in vitro	0	NULL	NULL	NULL	gw60_genetics_160_2_697_s_410	11861572	A high degree of conservation in this predicted binding site is thought to be required for MURA binding because MURA fails to bind  in vitro to the divergent left TIR of the apparently inactive  Mu5 transposon ( B ENITO and WALBOT 1997   ).	bind
39142	1	10535	6	13	NULL	NULL	NULL	HDL	GP		bind					SR-BI	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_29_20344_s_187	10400657	A high degree of correlation between HDL binding and CE-selective uptake is seen over the entire range of HDL binding (Fig.  2), indicating a tight correspondence between HDL binding to SR-BI and the subsequent transfer of HDL-CE into the cell.	bind
39143	2	10535	6	13	NULL	NULL	NULL	HDL-CE	GP		is transfered to					cell	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_29_20344_s_187	10400657	A high degree of correlation between HDL binding and CE-selective uptake is seen over the entire range of HDL binding (Fig.  2), indicating a tight correspondence between HDL binding to SR-BI and the subsequent transfer of HDL-CE into the cell.	bind
39144	3	10535	6	13	NULL	NULL	NULL	statement 1	Process		correlates with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_29_20344_s_187	10400657	A high degree of correlation between HDL binding and CE-selective uptake is seen over the entire range of HDL binding (Fig.  2), indicating a tight correspondence between HDL binding to SR-BI and the subsequent transfer of HDL-CE into the cell.	bind
48788	1	10535	7	NULL	NULL	0	NULL	HDL	NULL		bind	NULL				SR-BI	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_29_20344_s_187	10400657	A high degree of correlation between HDL binding and CE-selective uptake is seen over the entire range of HDL binding (Fig.  2), indicating a tight correspondence between HDL binding to SR-BI and the subsequent transfer of HDL-CE into the cell.	bind
48789	2	10535	7	NULL	NULL	0	NULL	HDL-CE	NULL		transfers to	NULL				cell	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_29_20344_s_187	10400657	A high degree of correlation between HDL binding and CE-selective uptake is seen over the entire range of HDL binding (Fig.  2), indicating a tight correspondence between HDL binding to SR-BI and the subsequent transfer of HDL-CE into the cell.	bind
48790	3	10535	7	NULL	NULL	0	NULL	statement 1	NULL		corresponds to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_29_20344_s_187	10400657	A high degree of correlation between HDL binding and CE-selective uptake is seen over the entire range of HDL binding (Fig.  2), indicating a tight correspondence between HDL binding to SR-BI and the subsequent transfer of HDL-CE into the cell.	bind
39147	1	10537	6	13	NULL	NULL	NULL	mGlu2 receptor	GP		is localized on					cell body of golgi cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_40_2_163_s_6	11114394	A high density of [3](2S,2'R,3'R)-2-(2'',3''-dicarboxycyclopropyl)glycine ([3]DCG-IV) binding sites were detected in the granular layer of the rat cerebellum, matching the localization of mGlu2 receptor on cell bodies and axon terminals of Golgi cells (  Mutel et al., 1998).	bind
39148	2	10537	6	13	NULL	NULL	NULL	mGlu2 receptor	GP		is localized on					axon terminals of golgi cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_40_2_163_s_6	11114394	A high density of [3](2S,2'R,3'R)-2-(2'',3''-dicarboxycyclopropyl)glycine ([3]DCG-IV) binding sites were detected in the granular layer of the rat cerebellum, matching the localization of mGlu2 receptor on cell bodies and axon terminals of Golgi cells (  Mutel et al., 1998).	bind
48791	1	10537	7	10	NULL	0	NULL	granular layer	NULL	 rat;;cerebellum	contains	NULL					NULL		(2S,2'R,3'R)-2-(2'',3''-dicarboxycyclopropyl)glycine DCG-IV) binding site		NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_40_2_163_s_6	11114394	A high density of [3](2S,2'R,3'R)-2-(2'',3''-dicarboxycyclopropyl)glycine ([3]DCG-IV) binding sites were detected in the granular layer of the rat cerebellum, matching the localization of mGlu2 receptor on cell bodies and axon terminals of Golgi cells (  Mutel et al., 1998).	bind
50297	2	10537	7	10	NULL	0	NULL	mGlu2 receptor	NULL		localize on	NULL				cell body on golgi cells	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_40_2_163_s_6	11114394	A high density of [3](2S,2'R,3'R)-2-(2'',3''-dicarboxycyclopropyl)glycine ([3]DCG-IV) binding sites were detected in the granular layer of the rat cerebellum, matching the localization of mGlu2 receptor on cell bodies and axon terminals of Golgi cells (  Mutel et al., 1998).	bind
50298	3	10537	7	10	NULL	0	NULL	mGlu2 receptor	NULL		localize on	NULL				axon terminals of Golgi cells	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_40_2_163_s_6	11114394	A high density of [3](2S,2'R,3'R)-2-(2'',3''-dicarboxycyclopropyl)glycine ([3]DCG-IV) binding sites were detected in the granular layer of the rat cerebellum, matching the localization of mGlu2 receptor on cell bodies and axon terminals of Golgi cells (  Mutel et al., 1998).	bind
39038	1	10539	6	13	NULL	NULL	NULL	high mobility group protein	GP		bind							long		CAG repeat tracts	NULL	Saccharomyces cerevisiae	NULL	NULL	NULL	NULL	gw70_jbiolchem_281_23_15735_s_1	16603770	A high mobility group protein binds to long CAG repeat tracts and establishes their chromatin organization in Saccharomyces cerevisiae.	bind
39151	2	10539	6	13	NULL	NULL	NULL	statement 1	Process		establishes					chromatin	Chromosome	organization of		long CAG repeat tracts	NULL	Saccharomyces cerevisiae	NULL	NULL	NULL	NULL	gw70_jbiolchem_281_23_15735_s_1	16603770	A high mobility group protein binds to long CAG repeat tracts and establishes their chromatin organization in Saccharomyces cerevisiae.	bind
48794	1	10539	7	10	NULL	0	NULL	high mobility group protein 	NULL		bind	NULL					NULL	long 		CAG repeat tracts	NULL	Saccharomyces cerevisiae	NULL	NULL	NULL	NULL	gw70_jbiolchem_281_23_15735_s_1	16603770	A high mobility group protein binds to long CAG repeat tracts and establishes their chromatin organization in Saccharomyces cerevisiae.	bind
48795	2	10539	7	10	NULL	0	NULL	statement 1	NULL		establishes	NULL				chromatin 	NULL	organization of		long CAG repeat tracts	NULL	Saccharomyces cerevisiae	NULL	NULL	NULL	NULL	gw70_jbiolchem_281_23_15735_s_1	16603770	A high mobility group protein binds to long CAG repeat tracts and establishes their chromatin organization in Saccharomyces cerevisiae.	bind
39039	1	10541	6	13	NULL	NULL	NULL	insulin-like growth factor II messenger RNA	NucleicAcid		acts as a marker for					anaplasia	Process				NULL	meningiomas	NULL	NULL	NULL	NULL	gw60_amjpathol_161_2_665_s_210	12163391	A high ratio of insulin-like growth factor II/insulin-like growth factor binding protein 2 messenger RNA as a marker for anaplasia in meningiomas.	bind
39040	2	10541	6	13	NULL	NULL	NULL	insulin-like growth factor binding protein 2 messenger RNA	NucleicAcid		acts as a marker for					anaplasia	Process				NULL	meningiomas	NULL	NULL	NULL	NULL	gw60_amjpathol_161_2_665_s_210	12163391	A high ratio of insulin-like growth factor II/insulin-like growth factor binding protein 2 messenger RNA as a marker for anaplasia in meningiomas.	bind
48796	1	10541	7	NULL	NULL	0	NULL	 insulin-like growth factor II/insulin-like growth factor binding protein 2 messenger RNA	NULL	high ratio of	marker for	NULL				anaplasia	NULL				NULL	meningiomas	0	NULL	NULL	NULL	gw60_amjpathol_161_2_665_s_210	12163391	A high ratio of insulin-like growth factor II/insulin-like growth factor binding protein 2 messenger RNA as a marker for anaplasia in meningiomas.	bind
39041	1	10542	6	13	NULL	NULL	NULL	FADD-DD	GP		bind					Fas-DD	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_46_36217_s_132	10952991	A high salt concentration virtually abolished the binding affinity of FADD-DD for Fas-DD.	bind
50246	2	10542	6	13	NULL	NULL	NULL	salt	Chemical	high concentration of	abolishes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_46_36217_s_132	10952991	A high salt concentration virtually abolished the binding affinity of FADD-DD for Fas-DD.	bind
48797	1	10542	7	10	NULL	0	NULL	FADD-DD	NULL		bind	NULL				Fas-DD	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_46_36217_s_132	10952991	A high salt concentration virtually abolished the binding affinity of FADD-DD for Fas-DD.	bind
48798	2	10542	7	10	NULL	0	NULL	salt	NULL	high concentration of	abolishes	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_46_36217_s_132	10952991	A high salt concentration virtually abolished the binding affinity of FADD-DD for Fas-DD.	bind
39042	1	10543	6	13	NULL	NULL	NULL	Sir1p	GP		bind					HMR a	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_15_1817_s_90	12897051	A high-affinity ORC-binding site contributes to silencing of and efficient  Sir1p binding to  HMR  a.	bind
39043	2	10543	6	13	NULL	NULL	NULL			high-affinity	contributes to				ORC-binding site	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_15_1817_s_90	12897051	A high-affinity ORC-binding site contributes to silencing of and efficient  Sir1p binding to  HMR  a.	bind
39044	3	10543	6	13	NULL	NULL	NULL			high-affinity	contributes to				ORC-binding site	statement 1	Process	silencing of 			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_15_1817_s_90	12897051	A high-affinity ORC-binding site contributes to silencing of and efficient  Sir1p binding to  HMR  a.	bind
48799	1	10543	7	NULL	NULL	0	NULL	Sir1p	NULL		bind	NULL				HMR a	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_17_15_1817_s_90	12897051	A high-affinity ORC-binding site contributes to silencing of and efficient  Sir1p binding to  HMR  a.	bind
48800	2	10543	7	10	NULL	0	NULL		NULL	high-affinity	silence	NULL			ORC-binding site	statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_15_1817_s_90	12897051	A high-affinity ORC-binding site contributes to silencing of and efficient  Sir1p binding to  HMR  a.	bind
48801	3	10543	7	10	NULL	0	NULL		NULL	high affinity 	contributes to	NULL	efficiently		ORC-binding site	statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_15_1817_s_90	12897051	A high-affinity ORC-binding site contributes to silencing of and efficient  Sir1p binding to  HMR  a.	bind
39152	1	10545	6	13	NULL	NULL	NULL	high-fat diet	Food		does not increase					IBAT	OrganismPart	growth of 			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_am-j-physiol_253_5-pt-2_3688276_s_4	3688276	A high-fat diet, fed isoenergetically  to the low-fat diet, did not increase the growth of IBAT and decreased  specific GDP binding in both strains.	bind
39153	2	10545	6	13	NULL	NULL	NULL	high-fat diet	Food		decreases					GDP	Chemical	specific;; binding of 			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_am-j-physiol_253_5-pt-2_3688276_s_4	3688276	A high-fat diet, fed isoenergetically  to the low-fat diet, did not increase the growth of IBAT and decreased  specific GDP binding in both strains.	bind
48802	1	10545	7	NULL	NULL	0	NULL	high-fat diet	NULL		does not increase	NULL				IBAT	NULL	growth of			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_am-j-physiol_253_5-pt-2_3688276_s_4	3688276	A high-fat diet, fed isoenergetically  to the low-fat diet, did not increase the growth of IBAT and decreased  specific GDP binding in both strains.	bind
48803	2	10545	7	10	NULL	0	NULL	high-fat diet	NULL		decrease	NULL				GDP	NULL	specific;;binding of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_am-j-physiol_253_5-pt-2_3688276_s_4	3688276	A high-fat diet, fed isoenergetically  to the low-fat diet, did not increase the growth of IBAT and decreased  specific GDP binding in both strains.	bind
39154	1	10546	6	13	NULL	NULL	NULL	SmpB	GP		bind			OB fold		tmRNA	NucleicAcid	Aquifex aeolicus	elbow region of the TLD		NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_11_3529_s_29	15972795	A high-resolution crystal structure of a complex containing SmpB and the TLD of tmRNA from  Aquifex aeolicus ( ) reveals that one side of the OB fold in SmpB binds to the elbow region of the TLD and stabilizes its D-loop in an extended conformation.	bind
39155	2	10546	6	13	NULL	NULL	NULL	statement 1	Process		stabilizes					tmRNA	NucleicAcid	Aquifex aeolicus	D-loop		NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_11_3529_s_29	15972795	A high-resolution crystal structure of a complex containing SmpB and the TLD of tmRNA from  Aquifex aeolicus ( ) reveals that one side of the OB fold in SmpB binds to the elbow region of the TLD and stabilizes its D-loop in an extended conformation.	bind
48804	1	10546	7	NULL	NULL	0	NULL	SmpB	NULL		complex with	NULL				tmRNA	NULL	Aquifex aeolicus	TLD		NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_11_3529_s_29	15972795	A high-resolution crystal structure of a complex containing SmpB and the TLD of tmRNA from  Aquifex aeolicus ( ) reveals that one side of the OB fold in SmpB binds to the elbow region of the TLD and stabilizes its D-loop in an extended conformation.	bind
48805	2	10546	7	10	NULL	0	NULL	SmpB			bind			OB fold		tmRNA		Aquifex aeolicus	elbow region of TLD		NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_11_3529_s_29	15972795	A high-resolution crystal structure of a complex containing SmpB and the TLD of tmRNA from  Aquifex aeolicus ( ) reveals that one side of the OB fold in SmpB binds to the elbow region of the TLD and stabilizes its D-loop in an extended conformation.	bind
48806	3	10546	7	10	NULL	0	NULL	statement 1			stabilizes					tmRNA		Aquifex aeolicus	D-loop		NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_11_3529_s_29	15972795	A high-resolution crystal structure of a complex containing SmpB and the TLD of tmRNA from  Aquifex aeolicus ( ) reveals that one side of the OB fold in SmpB binds to the elbow region of the TLD and stabilizes its D-loop in an extended conformation.	bind
39045	1	10548	6	13	NULL	NULL	NULL	small molecules	Chemical		bind					Bcl-XL	GP		hydrophobic BH3-binding groove		NULL		NULL	NULL	NULL	NULL	gw70_nature_435_7042_677_s_28	15902208	A high-throughput NMR-based method for lead compound discovery called 'SAR by  NMR'' 20 was used to screen a chemical library to identify small molecules that bind to the  hydrophobic BH3-binding groove of Bcl-XL.	bind
48807	1	10548	7	NULL	NULL	0	NULL	small molecules	NULL		bind	NULL				Bcl-XL	NULL		hydrophobic BH3-binding groove		NULL		0	NULL	NULL	NULL	gw70_nature_435_7042_677_s_28	15902208	A high-throughput NMR-based method for lead compound discovery called 'SAR by  NMR'' 20 was used to screen a chemical library to identify small molecules that bind to the  hydrophobic BH3-binding groove of Bcl-XL.	bind
39046	1	10549	6	13	NULL	NULL	NULL	gp120	GP		is a type of					human immunodeficiency virus envelope glycoprotein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_46_30443_s_106	9804811	A higher affinity ( K D 40-400 nM) has been reported for the binding of the human immunodeficiency virus envelope glycoprotein gp120 to its cell surface receptor CD4 ( 23).	bind
39047	2	10549	6	13	NULL	NULL	NULL	CD4	GP		is a type of					cell surface receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_46_30443_s_106	9804811	A higher affinity ( K D 40-400 nM) has been reported for the binding of the human immunodeficiency virus envelope glycoprotein gp120 to its cell surface receptor CD4 ( 23).	bind
39048	3	10549	6	13	NULL	NULL	NULL	gp120	GP		bind		high affinity			CD4	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_46_30443_s_106	9804811	A higher affinity ( K D 40-400 nM) has been reported for the binding of the human immunodeficiency virus envelope glycoprotein gp120 to its cell surface receptor CD4 ( 23).	bind
48808	1	10549	7	NULL	NULL	0	NULL	gp120	NULL		bind	NULL	high affinity			CD4	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_46_30443_s_106	9804811	A higher affinity ( K D 40-400 nM) has been reported for the binding of the human immunodeficiency virus envelope glycoprotein gp120 to its cell surface receptor CD4 ( 23).	bind
48809	2	10549	7	NULL	NULL	0	NULL	gp120	NULL		is a type of	NULL				human immunodeficiency virus envelope glycoprotein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_46_30443_s_106	9804811	A higher affinity ( K D 40-400 nM) has been reported for the binding of the human immunodeficiency virus envelope glycoprotein gp120 to its cell surface receptor CD4 ( 23).	bind
48810	3	10549	7	NULL	NULL	0	NULL	CD4	NULL		is a type of	NULL				cell surface receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_46_30443_s_106	9804811	A higher affinity ( K D 40-400 nM) has been reported for the binding of the human immunodeficiency virus envelope glycoprotein gp120 to its cell surface receptor CD4 ( 23).	bind
39049	1	10550	6	13	NULL	NULL	NULL	PD 158771	Chemical		bind		preferentially			D2L receptors	GP		D2 high affinity agonist binding site		NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_7_1197_s_292	10760362	A higher affinity was achieved when the D2L receptors were labeled with DA agonist [3]N-0437, suggesting that PD 158771 binds preferentially to the D2 high affinity agonist binding site.	bind
48811	1	10550	7	NULL	NULL	0	NULL	PD 158771	NULL		bind	NULL	preferentially			D2L receptor	NULL		D2 high affinity agonist binding site		NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_39_7_1197_s_292	10760362	A higher affinity was achieved when the D2L receptors were labeled with DA agonist [3]N-0437, suggesting that PD 158771 binds preferentially to the D2 high affinity agonist binding site.	bind
39156	1	10552	6	13	NULL	NULL	NULL	RMK	GP		bind		irreversibly			liver macromolecules	GP	mouse			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_mutat-res_119_1_6337321_s_5	6337321	A higher percentage  of RMK and MK became irreversibly bound to mouse-liver macromolecules  than to rat-liver macromolecules when incubated at 37 degrees C in the  presence of reduced nicotinamide adenine dinucleotide phosphate.	bind
39157	2	10552	6	13	NULL	NULL	NULL	MK	GP		bind		irreversibly			liver macromolecules	GP	mouse			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_mutat-res_119_1_6337321_s_5	6337321	A higher percentage  of RMK and MK became irreversibly bound to mouse-liver macromolecules  than to rat-liver macromolecules when incubated at 37 degrees C in the  presence of reduced nicotinamide adenine dinucleotide phosphate.	bind
39158	3	10552	6	13	NULL	NULL	NULL	RMK	GP		bind		irreversibly			liver macromolecules	GP	rat			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_mutat-res_119_1_6337321_s_5	6337321	A higher percentage  of RMK and MK became irreversibly bound to mouse-liver macromolecules  than to rat-liver macromolecules when incubated at 37 degrees C in the  presence of reduced nicotinamide adenine dinucleotide phosphate.	bind
39159	4	10552	6	13	NULL	NULL	NULL	MK	GP		bind		irreversibly			liver macromolecules	GP	rat			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_mutat-res_119_1_6337321_s_5	6337321	A higher percentage  of RMK and MK became irreversibly bound to mouse-liver macromolecules  than to rat-liver macromolecules when incubated at 37 degrees C in the  presence of reduced nicotinamide adenine dinucleotide phosphate.	bind
39160	5	10552	6	13	NULL	NULL	NULL	statement 1	Process		is greater than					statement 3	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_mutat-res_119_1_6337321_s_5	6337321	A higher percentage  of RMK and MK became irreversibly bound to mouse-liver macromolecules  than to rat-liver macromolecules when incubated at 37 degrees C in the  presence of reduced nicotinamide adenine dinucleotide phosphate.	bind
39161	6	10552	6	13	NULL	NULL	NULL	statement 5	Process		occurs in presence of					nicotinamide adenine dinucleotide phosphate	Chemical	reduced			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_mutat-res_119_1_6337321_s_5	6337321	A higher percentage  of RMK and MK became irreversibly bound to mouse-liver macromolecules  than to rat-liver macromolecules when incubated at 37 degrees C in the  presence of reduced nicotinamide adenine dinucleotide phosphate.	bind
39162	7	10552	6	13	NULL	NULL	NULL	statement 2	Process		is greater than					statement 4	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_mutat-res_119_1_6337321_s_5	6337321	A higher percentage  of RMK and MK became irreversibly bound to mouse-liver macromolecules  than to rat-liver macromolecules when incubated at 37 degrees C in the  presence of reduced nicotinamide adenine dinucleotide phosphate.	bind
39163	8	10552	6	13	NULL	NULL	NULL	statement 7	Process		occurs in presence of					nicotinamide adenine dinucleotide phosphate	Chemical	reduced			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_mutat-res_119_1_6337321_s_5	6337321	A higher percentage  of RMK and MK became irreversibly bound to mouse-liver macromolecules  than to rat-liver macromolecules when incubated at 37 degrees C in the  presence of reduced nicotinamide adenine dinucleotide phosphate.	bind
48813	1	10552	7	NULL	NULL	0	NULL	RMK 	NULL		bind	NULL	irreversibly			macromolecules	NULL	mouse-liver			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_mutat-res_119_1_6337321_s_5	6337321	A higher percentage  of RMK and MK became irreversibly bound to mouse-liver macromolecules  than to rat-liver macromolecules when incubated at 37 degrees C in the  presence of reduced nicotinamide adenine dinucleotide phosphate.	bind
48814	2	10552	7	NULL	NULL	0	NULL	MK	NULL		bind	NULL	irreversibly			macromolecules	NULL	mouse-liver			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_mutat-res_119_1_6337321_s_5	6337321	A higher percentage  of RMK and MK became irreversibly bound to mouse-liver macromolecules  than to rat-liver macromolecules when incubated at 37 degrees C in the  presence of reduced nicotinamide adenine dinucleotide phosphate.	bind
48815	3	10552	7	NULL	NULL	0	NULL	RMK	NULL		bind	NULL	irreversibly			macromolecules	NULL	rat-liver			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_mutat-res_119_1_6337321_s_5	6337321	A higher percentage  of RMK and MK became irreversibly bound to mouse-liver macromolecules  than to rat-liver macromolecules when incubated at 37 degrees C in the  presence of reduced nicotinamide adenine dinucleotide phosphate.	bind
48816	4	10552	7	NULL	NULL	0	NULL	MK	NULL		bind	NULL	irreversibly			macromolecules	NULL	rat-liver			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_mutat-res_119_1_6337321_s_5	6337321	A higher percentage  of RMK and MK became irreversibly bound to mouse-liver macromolecules  than to rat-liver macromolecules when incubated at 37 degrees C in the  presence of reduced nicotinamide adenine dinucleotide phosphate.	bind
48817	6	10552	7	10	NULL	0	NULL	statement 5			in presence of					nicotinamide adenine dinucleotide phosphate		reduced			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_mutat-res_119_1_6337321_s_5	6337321	A higher percentage  of RMK and MK became irreversibly bound to mouse-liver macromolecules  than to rat-liver macromolecules when incubated at 37 degrees C in the  presence of reduced nicotinamide adenine dinucleotide phosphate.	bind
48818	8	10552	7	10	NULL	0	NULL	statement 7			in presence of					nicotinamide adenine dinucleotide phosphate		reduced			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_mutat-res_119_1_6337321_s_5	6337321	A higher percentage  of RMK and MK became irreversibly bound to mouse-liver macromolecules  than to rat-liver macromolecules when incubated at 37 degrees C in the  presence of reduced nicotinamide adenine dinucleotide phosphate.	bind
48821	5	10552	7	10	NULL	0	NULL	statement 1		affinity of	is higher than					statement 3		affinity of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_mutat-res_119_1_6337321_s_5	6337321	A higher percentage  of RMK and MK became irreversibly bound to mouse-liver macromolecules  than to rat-liver macromolecules when incubated at 37 degrees C in the  presence of reduced nicotinamide adenine dinucleotide phosphate.	bind
48822	7	10552	7	10	NULL	0	NULL	statement 2		affinity of	is higher than					statement 4		affinity of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_mutat-res_119_1_6337321_s_5	6337321	A higher percentage  of RMK and MK became irreversibly bound to mouse-liver macromolecules  than to rat-liver macromolecules when incubated at 37 degrees C in the  presence of reduced nicotinamide adenine dinucleotide phosphate.	bind
39050	1	10553	6	13	NULL	NULL	NULL	Notch	GP		bind		cooperatively			RBP-jkappa	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_8_5106_s_394	16365048	A higher probability of activation could result from Notch binding to RBP-jkappa cooperatively when two RBP-jkappa molecules are properly positioned in proximity to each other.	bind
48823	1	10553	7	NULL	NULL	0	NULL	Notch	NULL		bind	NULL	cooperatively			RBP-jkappa	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_8_5106_s_394	16365048	A higher probability of activation could result from Notch binding to RBP-jkappa cooperatively when two RBP-jkappa molecules are properly positioned in proximity to each other.	bind
39051	1	10554	6	13	NULL	NULL	NULL	PACS-1	GP		is					phosphofurin acidic cluster sorting protein-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_21_2677_s_120	11069884	A highly conserved acidic cluster (AC) in the amino-proximal third of Nef (EEEE65) binds PACS-1 (phosphofurin acidic cluster sorting protein-1), the first identified member of a new family of coat proteins.	bind
39052	2	10554	6	13	NULL	NULL	NULL	PACS-1	GP		is a type of					coat protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_21_2677_s_120	11069884	A highly conserved acidic cluster (AC) in the amino-proximal third of Nef (EEEE65) binds PACS-1 (phosphofurin acidic cluster sorting protein-1), the first identified member of a new family of coat proteins.	bind
39053	3	10554	6	13	NULL	NULL	NULL	Nef	GP		bind			EEEE65		PACS-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_21_2677_s_120	11069884	A highly conserved acidic cluster (AC) in the amino-proximal third of Nef (EEEE65) binds PACS-1 (phosphofurin acidic cluster sorting protein-1), the first identified member of a new family of coat proteins.	bind
39054	4	10554	6	13	NULL	NULL	NULL	AC	GP		is 					acidic cluster	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_21_2677_s_120	11069884	A highly conserved acidic cluster (AC) in the amino-proximal third of Nef (EEEE65) binds PACS-1 (phosphofurin acidic cluster sorting protein-1), the first identified member of a new family of coat proteins.	bind
39055	5	10554	6	13	NULL	NULL	NULL	EEEE65	GP		is					highly conserved acidic cluster in the amino-proximal third	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_21_2677_s_120	11069884	A highly conserved acidic cluster (AC) in the amino-proximal third of Nef (EEEE65) binds PACS-1 (phosphofurin acidic cluster sorting protein-1), the first identified member of a new family of coat proteins.	bind
48827	1	10554	7	NULL	NULL	0	NULL	Nef	NULL		bind	NULL		amino-proximal EEEE65		PACS-1	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_14_21_2677_s_120	11069884	A highly conserved acidic cluster (AC) in the amino-proximal third of Nef (EEEE65) binds PACS-1 (phosphofurin acidic cluster sorting protein-1), the first identified member of a new family of coat proteins.	bind
48828	2	10554	7	NULL	NULL	0	NULL	Nef	NULL		is a type of	NULL		amino-proximal EEEE65		AC	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_14_21_2677_s_120	11069884	A highly conserved acidic cluster (AC) in the amino-proximal third of Nef (EEEE65) binds PACS-1 (phosphofurin acidic cluster sorting protein-1), the first identified member of a new family of coat proteins.	bind
48829	3	10554	7	NULL	NULL	0	NULL	AC	NULL		is	NULL				acidic cluster	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_14_21_2677_s_120	11069884	A highly conserved acidic cluster (AC) in the amino-proximal third of Nef (EEEE65) binds PACS-1 (phosphofurin acidic cluster sorting protein-1), the first identified member of a new family of coat proteins.	bind
48830	4	10554	7	NULL	NULL	0	NULL	PACS-1	NULL		is	NULL				phosphofurin acidic cluster sorting protein-1	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_14_21_2677_s_120	11069884	A highly conserved acidic cluster (AC) in the amino-proximal third of Nef (EEEE65) binds PACS-1 (phosphofurin acidic cluster sorting protein-1), the first identified member of a new family of coat proteins.	bind
48831	5	10554	7	NULL	NULL	0	NULL	PACS-1	NULL		is a type of	NULL				coat protein	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_14_21_2677_s_120	11069884	A highly conserved acidic cluster (AC) in the amino-proximal third of Nef (EEEE65) binds PACS-1 (phosphofurin acidic cluster sorting protein-1), the first identified member of a new family of coat proteins.	bind
39056	1	10556	6	13	NULL	NULL	NULL	HIV-1	Organism		bind			sulfate motif		CCR5	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_47_39493_s_1	16157597	A highly conserved arginine in gp120 governs HIV-1 binding to both syndecans and CCR5 via sulfated motifs.	bind
39057	2	10556	6	13	NULL	NULL	NULL	HIV-1	Organism		bind			sulfate motif		syndecan	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_47_39493_s_1	16157597	A highly conserved arginine in gp120 governs HIV-1 binding to both syndecans and CCR5 via sulfated motifs.	bind
39058	3	10556	6	13	NULL	NULL	NULL	gp120	GP	highly conserved	governs			arginine		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_47_39493_s_1	16157597	A highly conserved arginine in gp120 governs HIV-1 binding to both syndecans and CCR5 via sulfated motifs.	bind
39059	4	10556	6	13	NULL	NULL	NULL	gp120	GP	highly conserved	governs			arginine		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_47_39493_s_1	16157597	A highly conserved arginine in gp120 governs HIV-1 binding to both syndecans and CCR5 via sulfated motifs.	bind
48832	1	10556	7	NULL	NULL	0	NULL	HIV-1	NULL		bind	NULL		sulfated motif		syndecans	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_47_39493_s_1	16157597	A highly conserved arginine in gp120 governs HIV-1 binding to both syndecans and CCR5 via sulfated motifs.	bind
48833	2	10556	7	NULL	NULL	0	NULL	HIV-1	NULL		bind	NULL		sulfated motif		CCR5	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_47_39493_s_1	16157597	A highly conserved arginine in gp120 governs HIV-1 binding to both syndecans and CCR5 via sulfated motifs.	bind
48834	3	10556	7	10	NULL	0	NULL	gp120	NULL	highly conserved 	governs	NULL		arginine		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_47_39493_s_1	16157597	A highly conserved arginine in gp120 governs HIV-1 binding to both syndecans and CCR5 via sulfated motifs.	bind
48835	4	10556	7	10	NULL	0	NULL	gp120	NULL	highly conserved	governs	NULL		arginine		statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_47_39493_s_1	16157597	A highly conserved arginine in gp120 governs HIV-1 binding to both syndecans and CCR5 via sulfated motifs.	bind
39164	1	10558	6	13	NULL	NULL	NULL	HIV-1	Organism		bind					Syndecan	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_47_39493_s_146	16157597	A Highly Conserved Arginine in gp120 Mediates HIV-1 Binding to Syndecans --	bind
39165	2	10558	6	13	NULL	NULL	NULL	gp120	GP	highly conserved	mediates			arginine		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_47_39493_s_146	16157597	A Highly Conserved Arginine in gp120 Mediates HIV-1 Binding to Syndecans --	bind
48836	1	10558	7	NULL	NULL	0	NULL	HIV-1 	NULL		bind	NULL				Syndecans	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_47_39493_s_146	16157597	A Highly Conserved Arginine in gp120 Mediates HIV-1 Binding to Syndecans --	bind
48837	2	10558	7	10	NULL	0	NULL	gp120	NULL	highly conserved	mediates	NULL		Arginine		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_47_39493_s_146	16157597	A Highly Conserved Arginine in gp120 Mediates HIV-1 Binding to Syndecans --	bind
39844	1	10559	6	13	NULL	NULL	NULL	Rel/FkappaB family	GP	transcriptionally active	bind									CK1 element	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_24_14020_s_203	8662845	A highly conserved CK1/CK2 DNA sequence is present in this region and may be important in this activity, since a concatamer of this sequence has been shown to inhibit the basal transcription of a heterologous promoter and proteins from the transcriptionally active Rel/FkappaB family bind to the CK1 element ( 31).	bind
48838	1	10559	7	NULL	NULL	0	NULL		NULL	concatamer of	inhibit	NULL		highly conserved CK1/CK2 DNA sequence		heterologous promoter	NULL	basal transcription of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_24_14020_s_203	8662845	A highly conserved CK1/CK2 DNA sequence is present in this region and may be important in this activity, since a concatamer of this sequence has been shown to inhibit the basal transcription of a heterologous promoter and proteins from the transcriptionally active Rel/FkappaB family bind to the CK1 element ( 31).	bind
48840	2	10559	7	10	NULL	0	NULL	Rel/FkappaB family	NULL	transcriptionally active	bind	NULL					NULL			CK1 element	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_24_14020_s_203	8662845	A highly conserved CK1/CK2 DNA sequence is present in this region and may be important in this activity, since a concatamer of this sequence has been shown to inhibit the basal transcription of a heterologous promoter and proteins from the transcriptionally active Rel/FkappaB family bind to the CK1 element ( 31).	bind
39212	1	10560	6	13	NULL	NULL	NULL	S-layer proteins	GP	L. acidophilus	bind			C-terminus		cell wall	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_68_12_5943_s_20	12450814	A highly conserved domain was recently shown to mediate the binding of the S-layer protein subunits to the cell wall in the C-terminal part of the  L. acidophilus group S-layer proteins ( 49).	bind
48841	1	10560	7	NULL	NULL	0	NULL	S-layer protein	NULL	L. acidophilus	bind	NULL		 C-terminal subunit		cell wall	NULL				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_68_12_5943_s_20	12450814	A highly conserved domain was recently shown to mediate the binding of the S-layer protein subunits to the cell wall in the C-terminal part of the  L. acidophilus group S-layer proteins ( 49).	bind
39307	1	10561	6	13	NULL	NULL	NULL	SGT1	GP	eukaryotic	bind		specifically			HSP90	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_embo-j_25_9_16619029_s_2	16619029	A highly conserved eukaryotic protein SGT1 binds specifically to the molecular  chaperone, HSP90.	bind
39309	2	10561	6	13	NULL	NULL	NULL	HSP90	GP		is a type of					molecular chaperone	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_embo-j_25_9_16619029_s_2	16619029	A highly conserved eukaryotic protein SGT1 binds specifically to the molecular  chaperone, HSP90.	bind
48853	1	10561	7	10	NULL	0	NULL	 SGT1		eukaryotic	bind		specifically			HSP90					NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_embo-j_25_9_16619029_s_2	16619029	A highly conserved eukaryotic protein SGT1 binds specifically to the molecular  chaperone, HSP90.	bind
48855	2	10561	7	10	NULL	0	NULL	HSP90			is a type of					molecular chaperone					NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_embo-j_25_9_16619029_s_2	16619029	A highly conserved eukaryotic protein SGT1 binds specifically to the molecular  chaperone, HSP90.	bind
39845	1	10562	6	13	NULL	NULL	NULL	PKR kinase	GP	cellular	bind					RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_7_4419_s_250	9020165	A highly conserved lysine residue (Fig.  2) established as essential for the R-motif mediated RNA-binding activity of the cellular PKR kinase and the viral E3L protein ( 29,  30,  33) was substituted with glutamic acid in either any one, or all three, of the R copies in the ADAR splice variants.	bind
39846	2	10562	6	13	NULL	NULL	NULL	E3L protein	GP	viral	bind					RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_7_4419_s_250	9020165	A highly conserved lysine residue (Fig.  2) established as essential for the R-motif mediated RNA-binding activity of the cellular PKR kinase and the viral E3L protein ( 29,  30,  33) was substituted with glutamic acid in either any one, or all three, of the R copies in the ADAR splice variants.	bind
39847	3	10562	6	13	NULL	NULL	NULL				mediates			conserved lysine residue in R motif		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_7_4419_s_250	9020165	A highly conserved lysine residue (Fig.  2) established as essential for the R-motif mediated RNA-binding activity of the cellular PKR kinase and the viral E3L protein ( 29,  30,  33) was substituted with glutamic acid in either any one, or all three, of the R copies in the ADAR splice variants.	bind
39848	4	10562	6	13	NULL	NULL	NULL				mediates			conserved lysine residue in R motif		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_7_4419_s_250	9020165	A highly conserved lysine residue (Fig.  2) established as essential for the R-motif mediated RNA-binding activity of the cellular PKR kinase and the viral E3L protein ( 29,  30,  33) was substituted with glutamic acid in either any one, or all three, of the R copies in the ADAR splice variants.	bind
48856	1	10562	7	NULL	NULL	0	NULL	PKR kinase	NULL	cellular	bind	NULL				RNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_7_4419_s_250	9020165	A highly conserved lysine residue (Fig.  2) established as essential for the R-motif mediated RNA-binding activity of the cellular PKR kinase and the viral E3L protein ( 29,  30,  33) was substituted with glutamic acid in either any one, or all three, of the R copies in the ADAR splice variants.	bind
48857	2	10562	7	10	NULL	0	NULL	E3L protein	NULL	 viral	bind	NULL				RNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_7_4419_s_250	9020165	A highly conserved lysine residue (Fig.  2) established as essential for the R-motif mediated RNA-binding activity of the cellular PKR kinase and the viral E3L protein ( 29,  30,  33) was substituted with glutamic acid in either any one, or all three, of the R copies in the ADAR splice variants.	bind
48858	3	10562	7	NULL	NULL	0	NULL		NULL		mediates	NULL		 R-motif		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_7_4419_s_250	9020165	A highly conserved lysine residue (Fig.  2) established as essential for the R-motif mediated RNA-binding activity of the cellular PKR kinase and the viral E3L protein ( 29,  30,  33) was substituted with glutamic acid in either any one, or all three, of the R copies in the ADAR splice variants.	bind
48859	4	10562	7	NULL	NULL	0	NULL		NULL		mediates	NULL		R-motif		statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_7_4419_s_250	9020165	A highly conserved lysine residue (Fig.  2) established as essential for the R-motif mediated RNA-binding activity of the cellular PKR kinase and the viral E3L protein ( 29,  30,  33) was substituted with glutamic acid in either any one, or all three, of the R copies in the ADAR splice variants.	bind
48860	5	10562	7	NULL	NULL	0	NULL		NULL		is required for	NULL		highly conserved lysine residue		statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_7_4419_s_250	9020165	A highly conserved lysine residue (Fig.  2) established as essential for the R-motif mediated RNA-binding activity of the cellular PKR kinase and the viral E3L protein ( 29,  30,  33) was substituted with glutamic acid in either any one, or all three, of the R copies in the ADAR splice variants.	bind
48861	6	10562	7	NULL	NULL	0	NULL		NULL		is required for	NULL		highly conserved lysine residue		statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_7_4419_s_250	9020165	A highly conserved lysine residue (Fig.  2) established as essential for the R-motif mediated RNA-binding activity of the cellular PKR kinase and the viral E3L protein ( 29,  30,  33) was substituted with glutamic acid in either any one, or all three, of the R copies in the ADAR splice variants.	bind
39310	1	10563	6	13	NULL	NULL	NULL	antigen 85 complex proteins	GP	recombinant	bind					fibronectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_8_4521_s_145	9988684	A highly conserved motif among the antigen 85 complex proteins, FEWYYQ, was identified as an important sequence in the binding of recombinant 85 complex proteins to fibronectin ( 12).	bind
39311	2	10563	6	13	NULL	NULL	NULL	antigen 85 complex protein	GP		is important for			FEWYYQ		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_8_4521_s_145	9988684	A highly conserved motif among the antigen 85 complex proteins, FEWYYQ, was identified as an important sequence in the binding of recombinant 85 complex proteins to fibronectin ( 12).	bind
48862	1	10563	7	NULL	NULL	0	NULL	 antigen 85 complex protein	NULL	recombinant	bind	NULL				fibronectin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_8_4521_s_145	9988684	A highly conserved motif among the antigen 85 complex proteins, FEWYYQ, was identified as an important sequence in the binding of recombinant 85 complex proteins to fibronectin ( 12).	bind
48863	2	10563	7	NULL	NULL	0	NULL	antigen 85 complex protein	NULL		is required for	NULL		FEWYYQ		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_8_4521_s_145	9988684	A highly conserved motif among the antigen 85 complex proteins, FEWYYQ, was identified as an important sequence in the binding of recombinant 85 complex proteins to fibronectin ( 12).	bind
39312	1	10564	6	13	NULL	NULL	NULL	ETV6-NTRK3	GP		bind			NTRK3 C-terminal sequence		insulin receptor substrate-1	GP		phosphotyrosine binding domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_8_6225_s_1	14668342	A highly conserved NTRK3 C-terminal sequence in the ETV6-NTRK3 oncoprotein binds the phosphotyrosine binding domain of insulin receptor substrate-1: an essential interaction for transformation.	bind
50257	2	10564	6	13	NULL	NULL	NULL	statement 1	Process		is essential for					transformation	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_8_6225_s_1	14668342	A highly conserved NTRK3 C-terminal sequence in the ETV6-NTRK3 oncoprotein binds the phosphotyrosine binding domain of insulin receptor substrate-1: an essential interaction for transformation.	bind
50258	3	10564	6	13	NULL	NULL	NULL	ETV6-NTRK3	GP		is a type of					oncoprotein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_8_6225_s_1	14668342	A highly conserved NTRK3 C-terminal sequence in the ETV6-NTRK3 oncoprotein binds the phosphotyrosine binding domain of insulin receptor substrate-1: an essential interaction for transformation.	bind
48864	1	10564	7	NULL	NULL	0	NULL	ETV6-NTRK3	NULL		bind	NULL		highly conserved NTRK3 C-terminal sequence		insulin receptor substrate-1	NULL		 phosphotyrosine binding domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_8_6225_s_1	14668342	A highly conserved NTRK3 C-terminal sequence in the ETV6-NTRK3 oncoprotein binds the phosphotyrosine binding domain of insulin receptor substrate-1: an essential interaction for transformation.	bind
48865	2	10564	7	NULL	NULL	0	NULL	statement 1	NULL		is essential for	NULL				transformation	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_6225_s_1	14668342	A highly conserved NTRK3 C-terminal sequence in the ETV6-NTRK3 oncoprotein binds the phosphotyrosine binding domain of insulin receptor substrate-1: an essential interaction for transformation.	bind
48866	3	10564	7	NULL	NULL	0	NULL	ETV6-NTRK3	NULL		is a type of	NULL				oncoprotein	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_6225_s_1	14668342	A highly conserved NTRK3 C-terminal sequence in the ETV6-NTRK3 oncoprotein binds the phosphotyrosine binding domain of insulin receptor substrate-1: an essential interaction for transformation.	bind
39313	1	10566	6	13	NULL	NULL	NULL	RyR2	GP		is					cardiac muscle RyR	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_45_37941_s_150	16157601	A highly homologous protein (FKBP12.6) binds to the cardiac muscle RyR (known as RyR2) and stabilizes RyR2 in a similar manner ( ,  ).	bind
39314	2	10566	6	13	NULL	NULL	NULL	FKBP12.6	GP		bind					RyR2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_45_37941_s_150	16157601	A highly homologous protein (FKBP12.6) binds to the cardiac muscle RyR (known as RyR2) and stabilizes RyR2 in a similar manner ( ,  ).	bind
39315	3	10566	6	13	NULL	NULL	NULL	statement 2	Process		stabilizes					RyR2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_45_37941_s_150	16157601	A highly homologous protein (FKBP12.6) binds to the cardiac muscle RyR (known as RyR2) and stabilizes RyR2 in a similar manner ( ,  ).	bind
48867	1	10566	7	10	NULL	0	NULL	FKBP12.6	NULL		bind	NULL				RyR	NULL	cardiac muscle			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_45_37941_s_150	16157601	A highly homologous protein (FKBP12.6) binds to the cardiac muscle RyR (known as RyR2) and stabilizes RyR2 in a similar manner ( ,  ).	bind
48868	2	10566	7	NULL	NULL	0	NULL	statement 1	NULL		stabilizes	NULL				RyR2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_45_37941_s_150	16157601	A highly homologous protein (FKBP12.6) binds to the cardiac muscle RyR (known as RyR2) and stabilizes RyR2 in a similar manner ( ,  ).	bind
48869	3	10566	7	10	NULL	0	NULL	cardiac muscle RyR	NULL		is	NULL				RyR2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_45_37941_s_150	16157601	A highly homologous protein (FKBP12.6) binds to the cardiac muscle RyR (known as RyR2) and stabilizes RyR2 in a similar manner ( ,  ).	bind
39316	1	10567	6	13	NULL	NULL	NULL	Mcm4	GP	highly phosphorylated	accumulates on					chromatin	Chromosome				NULL	Xenopus egg extracts	NULL	NULL	NULL	NULL	gw70_genesdev_19_19_2295_s_85	16204181	A highly phosphorylated form of Mcm4 has been described and shown to accumulate on chromatin at the G1/S transition in  Xenopus egg extracts independently of Cdk2 activity (Pereverzeva et al. 2000 ).	bind
39317	2	10567	6	13	NULL	NULL	NULL	statement 1	Process		occurs during					G1/S transition	Process				NULL	Xenopus egg extracts	NULL	NULL	NULL	NULL	gw70_genesdev_19_19_2295_s_85	16204181	A highly phosphorylated form of Mcm4 has been described and shown to accumulate on chromatin at the G1/S transition in  Xenopus egg extracts independently of Cdk2 activity (Pereverzeva et al. 2000 ).	bind
39318	3	10567	6	13	NULL	NULL	NULL	statement 1	Process		is independent of					Cdk2	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_19_2295_s_85	16204181	A highly phosphorylated form of Mcm4 has been described and shown to accumulate on chromatin at the G1/S transition in  Xenopus egg extracts independently of Cdk2 activity (Pereverzeva et al. 2000 ).	bind
48870	1	10567	7	10	NULL	0	NULL	Mcm4	NULL	highly phosphorylated	accumulate on	NULL				chromatin	NULL				NULL	Xenopus egg extracts	NULL	NULL	NULL	NULL	gw70_genesdev_19_19_2295_s_85	16204181	A highly phosphorylated form of Mcm4 has been described and shown to accumulate on chromatin at the G1/S transition in  Xenopus egg extracts independently of Cdk2 activity (Pereverzeva et al. 2000 ).	bind
48871	2	10567	7	10	NULL	0	NULL	statement 1	NULL		is independent of	NULL				Cdk2 	NULL	activity of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_19_2295_s_85	16204181	A highly phosphorylated form of Mcm4 has been described and shown to accumulate on chromatin at the G1/S transition in  Xenopus egg extracts independently of Cdk2 activity (Pereverzeva et al. 2000 ).	bind
50259	3	10567	7	10	NULL	0	NULL	statement 1	NULL		occurs during	NULL				G1/S transition	NULL				NULL	Xenopus egg extracts	0	NULL	NULL	NULL	gw70_genesdev_19_19_2295_s_85	16204181	A highly phosphorylated form of Mcm4 has been described and shown to accumulate on chromatin at the G1/S transition in  Xenopus egg extracts independently of Cdk2 activity (Pereverzeva et al. 2000 ).	bind
39319	1	10568	6	13	NULL	NULL	NULL	CsrA	GP		bind					CsrB	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_18_5130_s_34	12193630	A highly repeated sequence element that is located in the loops of predicted CsrB hairpins and is related to the sequences involved in  glgCAP recognition sites ( 6) probably mediates the binding of CsrA to CsrB.	bind
39320	2	10568	6	13	NULL	NULL	NULL	CsrB hairpins	GP		mediates		probably		repeated sequence element	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_18_5130_s_34	12193630	A highly repeated sequence element that is located in the loops of predicted CsrB hairpins and is related to the sequences involved in  glgCAP recognition sites ( 6) probably mediates the binding of CsrA to CsrB.	bind
48872	1	10568	7	NULL	NULL	0	NULL	CsrA	NULL		bind	NULL				CsrB	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_18_5130_s_34	12193630	A highly repeated sequence element that is located in the loops of predicted CsrB hairpins and is related to the sequences involved in  glgCAP recognition sites ( 6) probably mediates the binding of CsrA to CsrB.	bind
48873	2	10568	7	NULL	NULL	0	NULL	CsrB hairpins	NULL		is related to	NULL			highly repeated sequence element in loops of	glgCAP	NULL		sequences involved in recognition site of		NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_18_5130_s_34	12193630	A highly repeated sequence element that is located in the loops of predicted CsrB hairpins and is related to the sequences involved in  glgCAP recognition sites ( 6) probably mediates the binding of CsrA to CsrB.	bind
48874	3	10568	7	NULL	NULL	0	NULL	statement 2	NULL		mediate	NULL	may			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_18_5130_s_34	12193630	A highly repeated sequence element that is located in the loops of predicted CsrB hairpins and is related to the sequences involved in  glgCAP recognition sites ( 6) probably mediates the binding of CsrA to CsrB.	bind
39849	1	10569	6	13	NULL	NULL	NULL	SecA subunit	GP		is a type of					ATPase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_20_15526_s_265	10809785	A highly similar model was proposed for the preprotein translocase of  E. coli, where the ATP-bound form of the SecA subunit, an ATPase, is membrane-embedded, while hydrolysis triggers release into the cytoplasm ( 31).	bind
39850	2	10569	6	13	NULL	NULL	NULL	ATP	Chemical		bind					preprotein translocase	GP	E. coli	SecA subunit		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_20_15526_s_265	10809785	A highly similar model was proposed for the preprotein translocase of  E. coli, where the ATP-bound form of the SecA subunit, an ATPase, is membrane-embedded, while hydrolysis triggers release into the cytoplasm ( 31).	bind
39851	3	10569	6	13	NULL	NULL	NULL	preprotein translocase	GP	E. coli	is embedded in			SecA subunit		membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_20_15526_s_265	10809785	A highly similar model was proposed for the preprotein translocase of  E. coli, where the ATP-bound form of the SecA subunit, an ATPase, is membrane-embedded, while hydrolysis triggers release into the cytoplasm ( 31).	bind
39852	4	10569	6	13	NULL	NULL	NULL	preprotein translocase	GP	E. coli	is released into 			SecA subunit		cytoplasm	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_20_15526_s_265	10809785	A highly similar model was proposed for the preprotein translocase of  E. coli, where the ATP-bound form of the SecA subunit, an ATPase, is membrane-embedded, while hydrolysis triggers release into the cytoplasm ( 31).	bind
39853	5	10569	6	13	NULL	NULL	NULL	hydrolysis	Process		triggers					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_20_15526_s_265	10809785	A highly similar model was proposed for the preprotein translocase of  E. coli, where the ATP-bound form of the SecA subunit, an ATPase, is membrane-embedded, while hydrolysis triggers release into the cytoplasm ( 31).	bind
48875	1	10569	7	10	NULL	0	NULL	ATP	NULL		bind	NULL				preprotein translocase	NULL	E. coli	SecA subunit		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_20_15526_s_265	10809785	A highly similar model was proposed for the preprotein translocase of  E. coli, where the ATP-bound form of the SecA subunit, an ATPase, is membrane-embedded, while hydrolysis triggers release into the cytoplasm ( 31).	bind
48876	2	10569	7	10	NULL	0	NULL	SecA subunit	NULL		is a type of	NULL				ATPase	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_20_15526_s_265	10809785	A highly similar model was proposed for the preprotein translocase of  E. coli, where the ATP-bound form of the SecA subunit, an ATPase, is membrane-embedded, while hydrolysis triggers release into the cytoplasm ( 31).	bind
48877	3	10569	7	10	NULL	0	NULL	preprotein translocase	NULL	E. coli	is embedded in	NULL		SecA subunit		membrane	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_20_15526_s_265	10809785	A highly similar model was proposed for the preprotein translocase of  E. coli, where the ATP-bound form of the SecA subunit, an ATPase, is membrane-embedded, while hydrolysis triggers release into the cytoplasm ( 31).	bind
48878	4	10569	7	10	NULL	0	NULL	preprotein translocase	NULL	E. coli	is released into	NULL		SecA subunit		cytoplasm	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_20_15526_s_265	10809785	A highly similar model was proposed for the preprotein translocase of  E. coli, where the ATP-bound form of the SecA subunit, an ATPase, is membrane-embedded, while hydrolysis triggers release into the cytoplasm ( 31).	bind
50260	5	10569	7	10	NULL	0	NULL	hydrolysis	NULL		triggers	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_20_15526_s_265	10809785	A highly similar model was proposed for the preprotein translocase of  E. coli, where the ATP-bound form of the SecA subunit, an ATPase, is membrane-embedded, while hydrolysis triggers release into the cytoplasm ( 31).	bind
39321	1	10570	6	13	NULL	NULL	NULL	streptococcal M protein family	GP		bind			variable region		C4BP	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_immunity_18_6_837_s_529	12818164	A highly variable region in members of the streptococcal M protein family binds the human complement regulator C4BP.	bind
39322	2	10570	6	13	NULL	NULL	NULL	C4BP	GP		is a type of					complement regulator	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_18_6_837_s_529	12818164	A highly variable region in members of the streptococcal M protein family binds the human complement regulator C4BP.	bind
48879	1	10570	7	NULL	NULL	0	NULL	streptococcal M protein family	NULL		bind	NULL		highly variable region		C4BP	NULL	human			NULL		NULL	NULL	NULL	NULL	gw60_immunity_18_6_837_s_529	12818164	A highly variable region in members of the streptococcal M protein family binds the human complement regulator C4BP.	bind
48880	2	10570	7	NULL	NULL	0	NULL	C4BP	NULL		is a type of	NULL				complement regulator	NULL				NULL		NULL	NULL	NULL	NULL	gw60_immunity_18_6_837_s_529	12818164	A highly variable region in members of the streptococcal M protein family binds the human complement regulator C4BP.	bind
39323	1	10571	6	13	NULL	NULL	NULL	Protamine	GP		bind					RyR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_7_2213_s_122	10888663	A Hill coefficient of >4 in a three-parameter Hill equation [f = (a x xb)/(cb + xb)] fit indicates that more than four molecules of protamine must bind to the RyR to induce block.	bind
39324	2	10571	6	13	NULL	NULL	NULL	statement 1	Process		induce					block	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_7_2213_s_122	10888663	A Hill coefficient of >4 in a three-parameter Hill equation [f = (a x xb)/(cb + xb)] fit indicates that more than four molecules of protamine must bind to the RyR to induce block.	bind
48881	1	10571	7	NULL	NULL	0	NULL	protamine	NULL		bind	NULL				RyR	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_7_2213_s_122	10888663	A Hill coefficient of >4 in a three-parameter Hill equation [f = (a x xb)/(cb + xb)] fit indicates that more than four molecules of protamine must bind to the RyR to induce block.	bind
48882	2	10571	7	NULL	NULL	0	NULL	statement 1	NULL		induce 	NULL				block	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_7_2213_s_122	10888663	A Hill coefficient of >4 in a three-parameter Hill equation [f = (a x xb)/(cb + xb)] fit indicates that more than four molecules of protamine must bind to the RyR to induce block.	bind
39325	1	10572	6	13	NULL	NULL	NULL	UmuD``C	GP		bind					M13 DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_18_10767_s_9	8631887	A Hill coefficient,  n  =  3, characterizes the binding of UmuD``C to M13 DNA and to  a 600 nucleotide DNA oligomer, suggesting that at least three protein  complexes may interact cooperatively when binding to DNA.	bind
39326	2	10572	6	13	NULL	NULL	NULL	UmuD``C	GP		bind					DNA oligomer	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_18_10767_s_9	8631887	A Hill coefficient,  n  =  3, characterizes the binding of UmuD``C to M13 DNA and to  a 600 nucleotide DNA oligomer, suggesting that at least three protein  complexes may interact cooperatively when binding to DNA.	bind
48883	1	10572	7	NULL	NULL	0	NULL	UmuD``C 	NULL		bind	NULL				M13 DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_18_10767_s_9	8631887	A Hill coefficient,  n  =  3, characterizes the binding of UmuD``C to M13 DNA and to  a 600 nucleotide DNA oligomer, suggesting that at least three protein  complexes may interact cooperatively when binding to DNA.	bind
48884	2	10572	7	10	NULL	0	NULL	UmuD``C	NULL		bind	NULL				DNA oligomer	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_18_10767_s_9	8631887	A Hill coefficient,  n  =  3, characterizes the binding of UmuD``C to M13 DNA and to  a 600 nucleotide DNA oligomer, suggesting that at least three protein  complexes may interact cooperatively when binding to DNA.	bind
39327	1	10576	6	13	NULL	NULL	NULL	CycT1	GP		bind			histidine-rich sequence in C terminus				unphosphorylated	CTD		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_6_748_s_34	12651893	A histidine-rich sequence in the C terminus of CycT1 then binds the unphosphorylated CTD.	bind
48892	1	10576	7	NULL	NULL	0	NULL	CycT1	NULL		bind	NULL		histidine-rich sequence in the C terminus			NULL	unphosphorylated	CTD		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_6_748_s_34	12651893	A histidine-rich sequence in the C terminus of CycT1 then binds the unphosphorylated CTD.	bind
39854	1	10577	6	13	NULL	NULL	NULL	phorbol ester	Chemical		bind					Munc13-1	GP		C1 domain		NULL		NULL	NULL	NULL	NULL	gw60_neuron_24_2_335_s_167	10571228	A histidine-to-lysine substitution at this position abolished phorbol ester binding to the C1 domain of Munc13-1 ( Betz et al. 1998  ), and other substitutions at this position abolished phorbol ester binding to protein kinase C  ( Kazanietz et al. 1995b  ).	bind
39855	2	10577	6	13	NULL	NULL	NULL	phorbol ester	Chemical		bind					protein kinase C	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_24_2_335_s_167	10571228	A histidine-to-lysine substitution at this position abolished phorbol ester binding to the C1 domain of Munc13-1 ( Betz et al. 1998  ), and other substitutions at this position abolished phorbol ester binding to protein kinase C  ( Kazanietz et al. 1995b  ).	bind
39856	3	10577	6	13	NULL	NULL	NULL	histidine	AminoAcid		is substituted with					lysine	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_neuron_24_2_335_s_167	10571228	A histidine-to-lysine substitution at this position abolished phorbol ester binding to the C1 domain of Munc13-1 ( Betz et al. 1998  ), and other substitutions at this position abolished phorbol ester binding to protein kinase C  ( Kazanietz et al. 1995b  ).	bind
39857	4	10577	6	13	NULL	NULL	NULL	statement 3	Process		abolishes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_24_2_335_s_167	10571228	A histidine-to-lysine substitution at this position abolished phorbol ester binding to the C1 domain of Munc13-1 ( Betz et al. 1998  ), and other substitutions at this position abolished phorbol ester binding to protein kinase C  ( Kazanietz et al. 1995b  ).	bind
48899	1	10577	7	NULL	NULL	0	NULL	phorbol ester	NULL		bind	NULL				Munc13-1	NULL		C1 domain		NULL		0	NULL	NULL	NULL	gw60_neuron_24_2_335_s_167	10571228	A histidine-to-lysine substitution at this position abolished phorbol ester binding to the C1 domain of Munc13-1 ( Betz et al. 1998  ), and other substitutions at this position abolished phorbol ester binding to protein kinase C  ( Kazanietz et al. 1995b  ).	bind
48900	4	10577	7	10	NULL	0	NULL	statement 2	NULL		abolishes	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuron_24_2_335_s_167	10571228	A histidine-to-lysine substitution at this position abolished phorbol ester binding to the C1 domain of Munc13-1 ( Betz et al. 1998  ), and other substitutions at this position abolished phorbol ester binding to protein kinase C  ( Kazanietz et al. 1995b  ).	bind
48901	3	10577	7	NULL	NULL	0	NULL	phorbol ester	NULL		bind	NULL				protein kinase C	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_24_2_335_s_167	10571228	A histidine-to-lysine substitution at this position abolished phorbol ester binding to the C1 domain of Munc13-1 ( Betz et al. 1998  ), and other substitutions at this position abolished phorbol ester binding to protein kinase C  ( Kazanietz et al. 1995b  ).	bind
50261	2	10577	7	10	NULL	0	NULL	histidine	NULL		is substituted to	NULL				lysine	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_24_2_335_s_167	10571228	A histidine-to-lysine substitution at this position abolished phorbol ester binding to the C1 domain of Munc13-1 ( Betz et al. 1998  ), and other substitutions at this position abolished phorbol ester binding to protein kinase C  ( Kazanietz et al. 1995b  ).	bind
39328	1	10579	6	13	NULL	NULL	NULL			homeotic mutation;;trithorax	impedes			SET domain		histone	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_nature_426_6962_78_s_252	14603321	A homeotic  mutation in the trithorax SET domain impedes histone binding.	bind
48903	1	10579	7	10	NULL	0	NULL		NULL	homeotic mutation;;trithorax	impede	NULL		SET domain		histone	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw70_nature_426_6962_78_s_252	14603321	A homeotic  mutation in the trithorax SET domain impedes histone binding.	bind
39329	1	10581	6	13	NULL	NULL	NULL	MPP11	GP	ribosome-associated fraction of	does not bind					Id1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_29_10064_s_117	16002468	A homolog of Id1 was not detected, suggesting that the ribosome-associated fraction of MPP11 was not bound to this transcription factor (see Introduction).	bind
39330	2	10581	6	13	NULL	NULL	NULL	Id1	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_29_10064_s_117	16002468	A homolog of Id1 was not detected, suggesting that the ribosome-associated fraction of MPP11 was not bound to this transcription factor (see Introduction).	bind
48906	1	10581	7	NULL	NULL	0	NULL	MPP11	NULL	ribosome-associated fraction of	does not bind	NULL				Id1	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_29_10064_s_117	16002468	A homolog of Id1 was not detected, suggesting that the ribosome-associated fraction of MPP11 was not bound to this transcription factor (see Introduction).	bind
50262	2	10581	7	10	NULL	0	NULL	Id1	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_29_10064_s_117	16002468	A homolog of Id1 was not detected, suggesting that the ribosome-associated fraction of MPP11 was not bound to this transcription factor (see Introduction).	bind
39331	1	10582	6	13	NULL	NULL	NULL	MarR 	GP		is a type of					repressor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_16_5131_s_67	10438794	A homologous MarR repressor binds salicylate and controls the expression of a global regulator, MarA, in  E. coli ( 14-16,  19).	bind
39332	2	10582	6	13	NULL	NULL	NULL	MarR	GP	homologous	bind					salicylate	Chemical				NULL	E.coli	NULL	NULL	NULL	NULL	gw60_jbacteriol_181_16_5131_s_67	10438794	A homologous MarR repressor binds salicylate and controls the expression of a global regulator, MarA, in  E. coli ( 14-16,  19).	bind
39333	3	10582	6	13	NULL	NULL	NULL	MarA	GP		is a type of					regulator	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_16_5131_s_67	10438794	A homologous MarR repressor binds salicylate and controls the expression of a global regulator, MarA, in  E. coli ( 14-16,  19).	bind
39334	4	10582	6	13	NULL	NULL	NULL	statement 1	Process		controls					MarA	GP	expression of			NULL	E.coli	NULL	NULL	NULL	NULL	gw60_jbacteriol_181_16_5131_s_67	10438794	A homologous MarR repressor binds salicylate and controls the expression of a global regulator, MarA, in  E. coli ( 14-16,  19).	bind
48907	1	10582	7	10	NULL	0	NULL	MarR	NULL	homologous	bind	NULL				salicylate	NULL				NULL	E.coli	NULL	NULL	NULL	NULL	gw60_jbacteriol_181_16_5131_s_67	10438794	A homologous MarR repressor binds salicylate and controls the expression of a global regulator, MarA, in  E. coli ( 14-16,  19).	bind
48908	2	10582	7	NULL	NULL	0	NULL	statement 1	NULL		controls	NULL				MarA	NULL	expression of			NULL	E.coli	0	NULL	NULL	NULL	gw60_jbacteriol_181_16_5131_s_67	10438794	A homologous MarR repressor binds salicylate and controls the expression of a global regulator, MarA, in  E. coli ( 14-16,  19).	bind
48909	3	10582	7	NULL	NULL	0	NULL	MarR	NULL		is a type of	NULL				repressor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_16_5131_s_67	10438794	A homologous MarR repressor binds salicylate and controls the expression of a global regulator, MarA, in  E. coli ( 14-16,  19).	bind
48910	4	10582	7	NULL	NULL	0	NULL	MarA	NULL		is a type of	NULL				global regulator	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_16_5131_s_67	10438794	A homologous MarR repressor binds salicylate and controls the expression of a global regulator, MarA, in  E. coli ( 14-16,  19).	bind
39335	1	10583	6	13	NULL	NULL	NULL	VirB	GP	Agrobacterium tumefaciens homologue	is essential for					Brucella suis	Organism	intracellular survival of 			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_2_865_s_237	11159979	A homologue of the  Agrobacterium tumefaciens VirB and  Bordetella pertussis Ptl type IV secretion systems is essential for intracellular survival of  Brucella suis.	bind
39336	2	10583	6	13	NULL	NULL	NULL	Ptl type IV secretion system	Process	Bordetella pertussis	is essential for					Brucella suis	Organism	intracellular survival of			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_69_2_865_s_237	11159979	A homologue of the  Agrobacterium tumefaciens VirB and  Bordetella pertussis Ptl type IV secretion systems is essential for intracellular survival of  Brucella suis.	bind
48911	1	10583	7	NULL	NULL	0	NULL	VirB	NULL	Agrobacterium tumefaciens homologue	is essential for	NULL				Brucella suis	NULL	intracellular survival of			NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_2_865_s_237	11159979	A homologue of the  Agrobacterium tumefaciens VirB and  Bordetella pertussis Ptl type IV secretion systems is essential for intracellular survival of  Brucella suis.	bind
48912	2	10583	7	NULL	NULL	0	NULL	Ptl type IV secretion systems	NULL	Bordetella pertussis	is essential for	NULL				Brucella suis	NULL	 intracellular survival of			NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_2_865_s_237	11159979	A homologue of the  Agrobacterium tumefaciens VirB and  Bordetella pertussis Ptl type IV secretion systems is essential for intracellular survival of  Brucella suis.	bind
39337	1	10584	6	13	NULL	NULL	NULL	progesterone	Chemical		bind					PR	GP		LBD		NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_63_5_1012_s_224	12695529	A homology model was created for the LBD of GR based on the X-ray crystal structure  of the progesterone bound LBD of PR (Williams and Sigler, 1998 ).	bind
48913	1	10584	7	NULL	NULL	0	NULL	progesterone 	NULL		bind	NULL				PR	NULL		LBD		NULL		0	NULL	NULL	NULL	gw70_molpharmacol_63_5_1012_s_224	12695529	A homology model was created for the LBD of GR based on the X-ray crystal structure  of the progesterone bound LBD of PR (Williams and Sigler, 1998 ).	bind
39352	1	10587	6	13	NULL	NULL	NULL	homopyrimidine third strand	NucleicAcid		contains					cytosine	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7295_s_33	7706270	A homopyrimidine third strand  containing cytosine and/or thymine binds to the purine strand in a  parallel orientation.	bind
39353	2	10587	6	13	NULL	NULL	NULL	homopyrimidine third strand	NucleicAcid		contains					thymine	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7295_s_33	7706270	A homopyrimidine third strand  containing cytosine and/or thymine binds to the purine strand in a  parallel orientation.	bind
39354	3	10587	6	13	NULL	NULL	NULL	statement 1	NucleicAcid		bind					purine strand	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7295_s_33	7706270	A homopyrimidine third strand  containing cytosine and/or thymine binds to the purine strand in a  parallel orientation.	bind
39355	4	10587	6	13	NULL	NULL	NULL	statement 2	NucleicAcid		bind					purine strand	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7295_s_33	7706270	A homopyrimidine third strand  containing cytosine and/or thymine binds to the purine strand in a  parallel orientation.	bind
39356	5	10587	6	13	NULL	NULL	NULL	statement 3	Process		occurs in					parallel orientation					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7295_s_33	7706270	A homopyrimidine third strand  containing cytosine and/or thymine binds to the purine strand in a  parallel orientation.	bind
39357	6	10587	6	13	NULL	NULL	NULL	statement 4	Process		occurs in					parallel orientation					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7295_s_33	7706270	A homopyrimidine third strand  containing cytosine and/or thymine binds to the purine strand in a  parallel orientation.	bind
48915	3	10587	7	10	NULL	0	NULL	statement 1	NULL		bind	NULL				purine strand	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7295_s_33	7706270	A homopyrimidine third strand  containing cytosine and/or thymine binds to the purine strand in a  parallel orientation.	bind
48916	5	10587	7	10	NULL	0	NULL	statement 3	NULL		occurs in	NULL				parallel orientation	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7295_s_33	7706270	A homopyrimidine third strand  containing cytosine and/or thymine binds to the purine strand in a  parallel orientation.	bind
48917	4	10587	7	10	NULL	0	NULL	statement 2	NULL		bind	NULL				purine strand	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7295_s_33	7706270	A homopyrimidine third strand  containing cytosine and/or thymine binds to the purine strand in a  parallel orientation.	bind
48918	6	10587	7	10	NULL	0	NULL	statement 4	NULL		occurs in	NULL				parallel orientation	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_13_7295_s_33	7706270	A homopyrimidine third strand  containing cytosine and/or thymine binds to the purine strand in a  parallel orientation.	bind
50263	1	10587	7	10	NULL	0	NULL	\thomopyrimidine third strand	NULL		contains	NULL				cytosine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_13_7295_s_33	7706270	A homopyrimidine third strand  containing cytosine and/or thymine binds to the purine strand in a  parallel orientation.	bind
50264	2	10587	7	10	NULL	0	NULL	homopyrimidine third strand	NULL		contains	NULL				thymine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_13_7295_s_33	7706270	A homopyrimidine third strand  containing cytosine and/or thymine binds to the purine strand in a  parallel orientation.	bind
39358	1	10588	6	13	NULL	NULL	NULL	RARs	GP		is a type of					retinoid receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_469_1_118_s_9	10708768	A HRE located between nucleotides -352 and -320 in the HIV long terminal repeat (LTR) binds retinoid receptors (RARs and RXRs) [  11 and   12].	bind
39359	2	10588	6	13	NULL	NULL	NULL	RXRs	GP		is a type of					retinoid receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_469_1_118_s_9	10708768	A HRE located between nucleotides -352 and -320 in the HIV long terminal repeat (LTR) binds retinoid receptors (RARs and RXRs) [  11 and   12].	bind
39360	3	10588	6	13	NULL	NULL	NULL	LTR	NucleicAcid		is					long terminal repeat	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_febslett_469_1_118_s_9	10708768	A HRE located between nucleotides -352 and -320 in the HIV long terminal repeat (LTR) binds retinoid receptors (RARs and RXRs) [  11 and   12].	bind
39361	4	10588	6	13	NULL	NULL	NULL	HIV LTR	NucleicAcid		bind				HRE (-352 to -320)	RAR	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_469_1_118_s_9	10708768	A HRE located between nucleotides -352 and -320 in the HIV long terminal repeat (LTR) binds retinoid receptors (RARs and RXRs) [  11 and   12].	bind
39362	5	10588	6	13	NULL	NULL	NULL	HIV LTR	NucleicAcid		bind				HRE (-352 to -320)	RXR	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_469_1_118_s_9	10708768	A HRE located between nucleotides -352 and -320 in the HIV long terminal repeat (LTR) binds retinoid receptors (RARs and RXRs) [  11 and   12].	bind
48920	2	10588	7	10	NULL	0	NULL	HIV LTR	NULL		bind	NULL			HRE (-352 to -320)	RARs	NULL				NULL		NULL	NULL	NULL	NULL	gw60_febslett_469_1_118_s_9	10708768	A HRE located between nucleotides -352 and -320 in the HIV long terminal repeat (LTR) binds retinoid receptors (RARs and RXRs) [  11 and   12].	bind
48921	3	10588	7	10	NULL	0	NULL	HIV LTR	NULL		bind	NULL			HRE (-352 to -320)	RXRs	NULL				NULL		NULL	NULL	NULL	NULL	gw60_febslett_469_1_118_s_9	10708768	A HRE located between nucleotides -352 and -320 in the HIV long terminal repeat (LTR) binds retinoid receptors (RARs and RXRs) [  11 and   12].	bind
48922	4	10588	7	NULL	NULL	0	NULL	RARs	NULL		is a type of	NULL				retinoid receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_469_1_118_s_9	10708768	A HRE located between nucleotides -352 and -320 in the HIV long terminal repeat (LTR) binds retinoid receptors (RARs and RXRs) [  11 and   12].	bind
48923	5	10588	7	NULL	NULL	0	NULL	RXRs	NULL		is a type of	NULL				retinoid receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_469_1_118_s_9	10708768	A HRE located between nucleotides -352 and -320 in the HIV long terminal repeat (LTR) binds retinoid receptors (RARs and RXRs) [  11 and   12].	bind
48924	1	10588	7	10	NULL	0	NULL	LTR			is					Long terminal repeat					NULL		NULL	NULL	NULL	NULL	gw60_febslett_469_1_118_s_9	10708768	A HRE located between nucleotides -352 and -320 in the HIV long terminal repeat (LTR) binds retinoid receptors (RARs and RXRs) [  11 and   12].	bind
39858	1	10589	6	13	NULL	NULL	NULL	HS species	Chemical		bind					FGF ligand	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_185_s_19	11786412	A HS species that binds both FGF ligand and RTK will act as a stimulator, whereas a HS that only binds FGF ligand will act as an inhibitor of signaling by sequestering the growth factor.	bind
39859	2	10589	6	13	NULL	NULL	NULL	HS species	Chemical		bind					RTK	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_160_1_185_s_19	11786412	A HS species that binds both FGF ligand and RTK will act as a stimulator, whereas a HS that only binds FGF ligand will act as an inhibitor of signaling by sequestering the growth factor.	bind
48925	1	10589	7	NULL	NULL	0	NULL	HS species	NULL		bind	NULL				FGF ligand	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_1_185_s_19	11786412	A HS species that binds both FGF ligand and RTK will act as a stimulator, whereas a HS that only binds FGF ligand will act as an inhibitor of signaling by sequestering the growth factor.	bind
48926	2	10589	7	NULL	NULL	0	NULL	HS species	NULL		bind	NULL				RTK	NULL				NULL		0	NULL	NULL	NULL	gw60_amjpathol_160_1_185_s_19	11786412	A HS species that binds both FGF ligand and RTK will act as a stimulator, whereas a HS that only binds FGF ligand will act as an inhibitor of signaling by sequestering the growth factor.	bind
39363	1	10591	6	13	NULL	NULL	NULL	endothelial cell membrane protein	GP	human	bind					Staphylococcus aureus	Organism				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_infectimmun_67_11_6130_s_584	10531276	A human endothelial cell membrane protein that binds  Staphylococcus aureus in vitro.	bind
48933	1	10591	7	NULL	NULL	0	NULL	endothelial cell membrane protein	NULL	human	bind	NULL				Staphylococcus aureus	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_infectimmun_67_11_6130_s_584	10531276	A human endothelial cell membrane protein that binds  Staphylococcus aureus in vitro.	bind
39860	1	10592	6	13	NULL	NULL	NULL	immunoglobulin G1 antibody	GP	human	bind		avidly			MUC1	GP	tumor-associated			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_am-j-pathol_160_5_12000712_s_1	12000712	A human immunoglobulin G1 antibody originating from an in vitro-selected Fab phage antibody binds avidly to tumor-associated MUC1 and is efficiently internalized..	bind
39861	2	10592	6	13	NULL	NULL	NULL	immunoglobulin G1 antibody	GP	human	originates from					Fab phage antibody	GP	in vitro-selected			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_am-j-pathol_160_5_12000712_s_1	12000712	A human immunoglobulin G1 antibody originating from an in vitro-selected Fab phage antibody binds avidly to tumor-associated MUC1 and is efficiently internalized..	bind
50265	3	10592	6	13	NULL	NULL	NULL	statement 1	Process		undergoes					internalization	Process	efficient			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_am-j-pathol_160_5_12000712_s_1	12000712	A human immunoglobulin G1 antibody originating from an in vitro-selected Fab phage antibody binds avidly to tumor-associated MUC1 and is efficiently internalized..	bind
48934	1	10592	7	10	NULL	0	NULL	immunoglobulin G1 antibody	NULL	human	originate from	NULL				Fab phage antibody	NULL	in vitro-selected 			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_am-j-pathol_160_5_12000712_s_1	12000712	A human immunoglobulin G1 antibody originating from an in vitro-selected Fab phage antibody binds avidly to tumor-associated MUC1 and is efficiently internalized..	bind
48935	2	10592	7	10	NULL	0	NULL	statement 1	NULL		bind	NULL	avidly			MUC1	NULL	tumor-associated			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_am-j-pathol_160_5_12000712_s_1	12000712	A human immunoglobulin G1 antibody originating from an in vitro-selected Fab phage antibody binds avidly to tumor-associated MUC1 and is efficiently internalized..	bind
48936	3	10592	7	10	NULL	0	NULL	statement 2	NULL		undergoes	NULL				internalization	NULL	efficient			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_am-j-pathol_160_5_12000712_s_1	12000712	A human immunoglobulin G1 antibody originating from an in vitro-selected Fab phage antibody binds avidly to tumor-associated MUC1 and is efficiently internalized..	bind
39364	1	10593	6	13	NULL	NULL	NULL	Rabin8	GP	human	bind					Rab8	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_methods-enzymol_403_1_16473595_s_5	16473595	A human protein (Rabin8) and its rat equivalent (Rabin3)  were found to bind Rab8 and function as nucleotide exchange factors for  Rab8 but not for Rab3A and Rab5.	bind
39365	2	10593	6	13	NULL	NULL	NULL	Rabin3	GP	rat	bind					Rab8	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_methods-enzymol_403_1_16473595_s_5	16473595	A human protein (Rabin8) and its rat equivalent (Rabin3)  were found to bind Rab8 and function as nucleotide exchange factors for  Rab8 but not for Rab3A and Rab5.	bind
39366	3	10593	6	13	NULL	NULL	NULL	statement 1	GP		function as					Rab8	GP	nucleotide exchange factor for			NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_methods-enzymol_403_1_16473595_s_5	16473595	A human protein (Rabin8) and its rat equivalent (Rabin3)  were found to bind Rab8 and function as nucleotide exchange factors for  Rab8 but not for Rab3A and Rab5.	bind
39367	4	10593	6	13	NULL	NULL	NULL	statement 2	GP		function as					Rab8	GP	nucleotide exchange factor for			NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_methods-enzymol_403_1_16473595_s_5	16473595	A human protein (Rabin8) and its rat equivalent (Rabin3)  were found to bind Rab8 and function as nucleotide exchange factors for  Rab8 but not for Rab3A and Rab5.	bind
39368	5	10593	6	13	NULL	NULL	NULL	statement 1	GP		does not function as					Rab3A	GP	nucleotide exchange factor for			NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_methods-enzymol_403_1_16473595_s_5	16473595	A human protein (Rabin8) and its rat equivalent (Rabin3)  were found to bind Rab8 and function as nucleotide exchange factors for  Rab8 but not for Rab3A and Rab5.	bind
39369	6	10593	6	13	NULL	NULL	NULL	statement 1	GP		does not function as					Rab5	GP	nucleotide exchange factor for			NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_methods-enzymol_403_1_16473595_s_5	16473595	A human protein (Rabin8) and its rat equivalent (Rabin3)  were found to bind Rab8 and function as nucleotide exchange factors for  Rab8 but not for Rab3A and Rab5.	bind
39370	7	10593	6	13	NULL	NULL	NULL	statement 2	GP		does not function as					Rab3A	GP	nucleotide exchange factor for			NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_methods-enzymol_403_1_16473595_s_5	16473595	A human protein (Rabin8) and its rat equivalent (Rabin3)  were found to bind Rab8 and function as nucleotide exchange factors for  Rab8 but not for Rab3A and Rab5.	bind
39371	8	10593	6	13	NULL	NULL	NULL	statement 2	GP		does not function as					Rab5	GP	nucleotide exchange factor for			NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_methods-enzymol_403_1_16473595_s_5	16473595	A human protein (Rabin8) and its rat equivalent (Rabin3)  were found to bind Rab8 and function as nucleotide exchange factors for  Rab8 but not for Rab3A and Rab5.	bind
48937	1	10593	7	NULL	NULL	0	NULL	Rabin8	NULL	human	bind	NULL				Rab8	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_methods-enzymol_403_1_16473595_s_5	16473595	A human protein (Rabin8) and its rat equivalent (Rabin3)  were found to bind Rab8 and function as nucleotide exchange factors for  Rab8 but not for Rab3A and Rab5.	bind
48938	2	10593	7	NULL	NULL	0	NULL	Rabin3	NULL	rat	bind	NULL				Rab8	NULL				NULL		0	NULL	NULL	NULL	abs-batch0600-0619_methods-enzymol_403_1_16473595_s_5	16473595	A human protein (Rabin8) and its rat equivalent (Rabin3)  were found to bind Rab8 and function as nucleotide exchange factors for  Rab8 but not for Rab3A and Rab5.	bind
48939	3	10593	7	NULL	NULL	0	NULL	statement 1	NULL		function as	NULL				Rab8	NULL	nucleotide exchange factors for			NULL		0	NULL	NULL	NULL	abs-batch0600-0619_methods-enzymol_403_1_16473595_s_5	16473595	A human protein (Rabin8) and its rat equivalent (Rabin3)  were found to bind Rab8 and function as nucleotide exchange factors for  Rab8 but not for Rab3A and Rab5.	bind
48940	4	10593	7	NULL	NULL	0	NULL	statement 2	NULL		function as	NULL				Rab8	NULL	nucleotide exchange factors for			NULL		0	NULL	NULL	NULL	abs-batch0600-0619_methods-enzymol_403_1_16473595_s_5	16473595	A human protein (Rabin8) and its rat equivalent (Rabin3)  were found to bind Rab8 and function as nucleotide exchange factors for  Rab8 but not for Rab3A and Rab5.	bind
48941	5	10593	7	NULL	NULL	0	NULL	statement 1	NULL		does not function as	NULL				Rab3A	NULL	nucleotide exchange factors for			NULL		0	NULL	NULL	NULL	abs-batch0600-0619_methods-enzymol_403_1_16473595_s_5	16473595	A human protein (Rabin8) and its rat equivalent (Rabin3)  were found to bind Rab8 and function as nucleotide exchange factors for  Rab8 but not for Rab3A and Rab5.	bind
48942	6	10593	7	NULL	NULL	0	NULL	statement 2	NULL		does not function as	NULL				Rab3A	NULL	nucleotide exchange factors for			NULL		0	NULL	NULL	NULL	abs-batch0600-0619_methods-enzymol_403_1_16473595_s_5	16473595	A human protein (Rabin8) and its rat equivalent (Rabin3)  were found to bind Rab8 and function as nucleotide exchange factors for  Rab8 but not for Rab3A and Rab5.	bind
48943	7	10593	7	NULL	NULL	0	NULL	statement 1	NULL		does not function as	NULL				Rab5	NULL	nucleotide exchange factors for			NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_methods-enzymol_403_1_16473595_s_5	16473595	A human protein (Rabin8) and its rat equivalent (Rabin3)  were found to bind Rab8 and function as nucleotide exchange factors for  Rab8 but not for Rab3A and Rab5.	bind
48944	8	10593	7	NULL	NULL	0	NULL	statement 2	NULL		does not function as	NULL				Rab5	NULL	nucleotide exchange factors for			NULL		0	NULL	NULL	NULL	abs-batch0600-0619_methods-enzymol_403_1_16473595_s_5	16473595	A human protein (Rabin8) and its rat equivalent (Rabin3)  were found to bind Rab8 and function as nucleotide exchange factors for  Rab8 but not for Rab3A and Rab5.	bind
39387	1	10594	6	13	NULL	NULL	NULL	protein	GP	human	contains								cold shock domain		NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_269_19_8188694_s_1	8188694	A human protein containing a "`cold"` shock domain binds specifically to H-DNA upstream from the human gamma-globin genes..	bind
39388	2	10594	6	13	NULL	NULL	NULL	statement 1	GP		bind		specifically			gamma globin genes	GP	human		H-DNA upstream from	NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_269_19_8188694_s_1	8188694	A human protein containing a "`cold"` shock domain binds specifically to H-DNA upstream from the human gamma-globin genes..	bind
48945	1	10594	7	10	NULL	0	NULL	protein		human	bind		specifically	cold shock domain		H-DNA				upstream from the human gamma-globin genes	NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_269_19_8188694_s_1	8188694	A human protein containing a "`cold"` shock domain binds specifically to H-DNA upstream from the human gamma-globin genes..	bind
39389	1	10595	6	13	NULL	NULL	NULL	protein	GP	human	interferes with					ras	GP	function of			NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_6_773_s_409	9208849	A human protein selected for interference with ras function interacts directly with ras and competes with raf1.	bind
39390	2	10595	6	13	NULL	NULL	NULL	statement 1	GP		interacts		directly			ras	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_6_773_s_409	9208849	A human protein selected for interference with ras function interacts directly with ras and competes with raf1.	bind
39391	3	10595	6	13	NULL	NULL	NULL	statement 1	GP		competes with					raf1	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_6_6_773_s_409	9208849	A human protein selected for interference with ras function interacts directly with ras and competes with raf1.	bind
48946	1	10595	7	NULL	NULL	0	NULL	 protein	NULL	human	interferes with	NULL				 ras 	NULL	function of			NULL		0	NULL	NULL	NULL	gw60_immunity_6_6_773_s_409	9208849	A human protein selected for interference with ras function interacts directly with ras and competes with raf1.	bind
48947	2	10595	7	NULL	NULL	0	NULL	statement 1	NULL		interacts with	NULL	directly			ras	NULL				NULL		0	NULL	NULL	NULL	gw60_immunity_6_6_773_s_409	9208849	A human protein selected for interference with ras function interacts directly with ras and competes with raf1.	bind
48948	3	10595	7	NULL	NULL	0	NULL	statement 1	NULL		compete with	NULL				raf1	NULL				NULL		0	NULL	NULL	NULL	gw60_immunity_6_6_773_s_409	9208849	A human protein selected for interference with ras function interacts directly with ras and competes with raf1.	bind
39392	1	10596	6	13	NULL	NULL	NULL	AMP	Chemical		bind								C1 subunit		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_20_19737_s_246	15767255	A hybrid tetramer of FBPase that constrains AMP binding to subunits C1 and C2, however, exhibits noncooperative inhibition, even though it undergoes a quaternary transition ( ).	bind
39393	2	10596	6	13	NULL	NULL	NULL	AMP	Chemical		bind								C2 subunit		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_20_19737_s_246	15767255	A hybrid tetramer of FBPase that constrains AMP binding to subunits C1 and C2, however, exhibits noncooperative inhibition, even though it undergoes a quaternary transition ( ).	bind
39394	3	10596	6	13	NULL	NULL	NULL	FBPase	GP	hybrid tetramer	constrains					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_20_19737_s_246	15767255	A hybrid tetramer of FBPase that constrains AMP binding to subunits C1 and C2, however, exhibits noncooperative inhibition, even though it undergoes a quaternary transition ( ).	bind
39395	4	10596	6	13	NULL	NULL	NULL	FBPase	GP	hybrid tetramer	constrains					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_20_19737_s_246	15767255	A hybrid tetramer of FBPase that constrains AMP binding to subunits C1 and C2, however, exhibits noncooperative inhibition, even though it undergoes a quaternary transition ( ).	bind
39399	5	10596	6	13	NULL	NULL	NULL	FBPase	GP	hybrid tetramer	undergoes a					quaternary transition	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_20_19737_s_246	15767255	A hybrid tetramer of FBPase that constrains AMP binding to subunits C1 and C2, however, exhibits noncooperative inhibition, even though it undergoes a quaternary transition ( ).	bind
48949	1	10596	7	NULL	NULL	0	NULL	AMP	NULL		bind	NULL					NULL		C1 subunit		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_19737_s_246	15767255	A hybrid tetramer of FBPase that constrains AMP binding to subunits C1 and C2, however, exhibits noncooperative inhibition, even though it undergoes a quaternary transition ( ).	bind
48950	2	10596	7	NULL	NULL	0	NULL	AMP	NULL		bind	NULL					NULL		C2 subunit		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_19737_s_246	15767255	A hybrid tetramer of FBPase that constrains AMP binding to subunits C1 and C2, however, exhibits noncooperative inhibition, even though it undergoes a quaternary transition ( ).	bind
48951	3	10596	7	NULL	NULL	0	NULL	FBPase	NULL	 hybrid tetramer of	constrains	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_19737_s_246	15767255	A hybrid tetramer of FBPase that constrains AMP binding to subunits C1 and C2, however, exhibits noncooperative inhibition, even though it undergoes a quaternary transition ( ).	bind
48952	4	10596	7	NULL	NULL	0	NULL	FBPase	NULL	hybrid tetramer of	constrains	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_19737_s_246	15767255	A hybrid tetramer of FBPase that constrains AMP binding to subunits C1 and C2, however, exhibits noncooperative inhibition, even though it undergoes a quaternary transition ( ).	bind
48953	5	10596	7	NULL	NULL	0	NULL	FBPase	NULL	hybrid tetramer of 	undergoes	NULL				quaternary transition	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_19737_s_246	15767255	A hybrid tetramer of FBPase that constrains AMP binding to subunits C1 and C2, however, exhibits noncooperative inhibition, even though it undergoes a quaternary transition ( ).	bind
39862	1	10598	6	13	NULL	NULL	NULL	IkappaBalpha	GP		forms			SRR		IkappaBbeta	GP	hybrid protein with			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_7_3048_s_222	15024091	A hydrid IkappaB protein containing the SRR of IkappaBalpha and the rest of IkappaBbeta binds poorly with kappaB-Ras (lane 3).	bind
39863	2	10598	6	13	NULL	NULL	NULL	statement 1	GP		bind		poorly			kappaB-Ras	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_7_3048_s_222	15024091	A hydrid IkappaB protein containing the SRR of IkappaBalpha and the rest of IkappaBbeta binds poorly with kappaB-Ras (lane 3).	bind
48955	2	10598	7	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL	poorly			kappaB-Ras	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_7_3048_s_222	15024091	A hydrid IkappaB protein containing the SRR of IkappaBalpha and the rest of IkappaBbeta binds poorly with kappaB-Ras (lane 3).	bind
48956	1	10598	7	10	NULL	0	NULL	IkappaBalpha	NULL		forms	NULL		SRR		IkappaBbeta	NULL	hybrid protein with			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_7_3048_s_222	15024091	A hydrid IkappaB protein containing the SRR of IkappaBalpha and the rest of IkappaBbeta binds poorly with kappaB-Ras (lane 3).	bind
39400	1	10599	6	13	NULL	NULL	NULL	FKBP12-rapamycin	GP		bind					TOR1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_46_27531_s_160	7499212	A hydrophobic  substitution of an FKBP12 acidic surface residue, D48V, had only a  minor 2-4-fold effect on FKBP12-rapamycin binding to TOR1 or TOR2 ( Fig. 5,  A  and  B).	bind
39401	2	10599	6	13	NULL	NULL	NULL	FKBP12-rapamycin	GP		bind					TOR2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_46_27531_s_160	7499212	A hydrophobic  substitution of an FKBP12 acidic surface residue, D48V, had only a  minor 2-4-fold effect on FKBP12-rapamycin binding to TOR1 or TOR2 ( Fig. 5,  A  and  B).	bind
39864	3	10599	6	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_46_27531_s_160	7499212	A hydrophobic  substitution of an FKBP12 acidic surface residue, D48V, had only a  minor 2-4-fold effect on FKBP12-rapamycin binding to TOR1 or TOR2 ( Fig. 5,  A  and  B).	bind
39865	4	10599	6	13	NULL	NULL	NULL	FKBP12	GP	hydrophobic substitution of 	effects		minor	acidic surface residue;; D48V		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_46_27531_s_160	7499212	A hydrophobic  substitution of an FKBP12 acidic surface residue, D48V, had only a  minor 2-4-fold effect on FKBP12-rapamycin binding to TOR1 or TOR2 ( Fig. 5,  A  and  B).	bind
39866	5	10599	6	13	NULL	NULL	NULL	FKBP12	GP	hydrophobic substitution of	effects		minor	acidic surface residue;; D48V		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_46_27531_s_160	7499212	A hydrophobic  substitution of an FKBP12 acidic surface residue, D48V, had only a  minor 2-4-fold effect on FKBP12-rapamycin binding to TOR1 or TOR2 ( Fig. 5,  A  and  B).	bind
48957	1	10599	7	NULL	NULL	0	NULL	FKBP12-rapamycin	NULL		bind	NULL				TOR1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_46_27531_s_160	7499212	A hydrophobic  substitution of an FKBP12 acidic surface residue, D48V, had only a  minor 2-4-fold effect on FKBP12-rapamycin binding to TOR1 or TOR2 ( Fig. 5,  A  and  B).	bind
48958	2	10599	7	NULL	NULL	0	NULL	FKBP12-rapamycin	NULL		bind	NULL				TOR2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_46_27531_s_160	7499212	A hydrophobic  substitution of an FKBP12 acidic surface residue, D48V, had only a  minor 2-4-fold effect on FKBP12-rapamycin binding to TOR1 or TOR2 ( Fig. 5,  A  and  B).	bind
48959	3	10599	7	10	NULL	0	NULL	FKBP12	NULL	hydrophobic substitution of	effects	NULL	minor	acidic surface residue;;D48V		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_46_27531_s_160	7499212	A hydrophobic  substitution of an FKBP12 acidic surface residue, D48V, had only a  minor 2-4-fold effect on FKBP12-rapamycin binding to TOR1 or TOR2 ( Fig. 5,  A  and  B).	bind
48960	4	10599	7	10	NULL	0	NULL	 FKBP12	NULL	hydrophobic substitution of	effects	NULL	minor	acidic surface residue;;D48V		statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_46_27531_s_160	7499212	A hydrophobic  substitution of an FKBP12 acidic surface residue, D48V, had only a  minor 2-4-fold effect on FKBP12-rapamycin binding to TOR1 or TOR2 ( Fig. 5,  A  and  B).	bind
57695	5	10599	7	10	NULL	0	NULL	statement 1			is an alternative to					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_46_27531_s_160	7499212	A hydrophobic  substitution of an FKBP12 acidic surface residue, D48V, had only a  minor 2-4-fold effect on FKBP12-rapamycin binding to TOR1 or TOR2 ( Fig. 5,  A  and  B).	bind
39402	1	10600	6	13	NULL	NULL	NULL	Cdc42	GP	geranylgeranyl moiety of	bind					membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_19_15776_s_223	11278313	A hydrophobic pocket in rhoGDI surrounds the membrane-binding geranylgeranyl moiety of Cdc42, thus leading to membrane release.	bind
39403	2	10600	6	13	NULL	NULL	NULL	rhoGDI	GP		surrounds			hydrophobic pocket		statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_19_15776_s_223	11278313	A hydrophobic pocket in rhoGDI surrounds the membrane-binding geranylgeranyl moiety of Cdc42, thus leading to membrane release.	bind
39404	3	10600	6	13	NULL	NULL	NULL	statement 2	Process		leads to					membrane	CellComponent	release of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_19_15776_s_223	11278313	A hydrophobic pocket in rhoGDI surrounds the membrane-binding geranylgeranyl moiety of Cdc42, thus leading to membrane release.	bind
48961	2	10600	7	NULL	NULL	0	NULL	rhoGDI	NULL		surrounds	NULL		hydrophobic pocket		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_19_15776_s_223	11278313	A hydrophobic pocket in rhoGDI surrounds the membrane-binding geranylgeranyl moiety of Cdc42, thus leading to membrane release.	bind
48962	1	10600	7	NULL	NULL	0	NULL	Cdc42	NULL	geranylgeranyl moiety of	bind	NULL				membrane	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_19_15776_s_223	11278313	A hydrophobic pocket in rhoGDI surrounds the membrane-binding geranylgeranyl moiety of Cdc42, thus leading to membrane release.	bind
48963	3	10600	7	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				membrane	NULL	release of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_19_15776_s_223	11278313	A hydrophobic pocket in rhoGDI surrounds the membrane-binding geranylgeranyl moiety of Cdc42, thus leading to membrane release.	bind
47133	1	10601	5	13	NULL	NULL	NULL	IRS1	GP		bind			-6 to -8 residues N-terminal to the phosphotyrosine					NP XpY motifs		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_6_4962_s_110	14607833	A hydrophobic residue at position -5 and a proline at -2 are crucial for the Shc PTB domain, but the amino acids from -6 to -8 residues N-terminal to the phosphotyrosine are important for IRS1 binding to the NP XpY motifs.	bind
39867	1	10601	6	NULL	NULL	0	NULL	IRS1	NULL		bind	NULL		\t-6 to -8 residues N-terminal to phosphotyrosine \t		Shc	NULL		NP XpY motifs		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_6_4962_s_110	14607833	A hydrophobic residue at position -5 and a proline at -2 are crucial for the Shc PTB domain, but the amino acids from -6 to -8 residues N-terminal to the phosphotyrosine are important for IRS1 binding to the NP XpY motifs.	bind
47135	1	10602	5	13	NULL	NULL	NULL	HslU	GP		bind			hydrophobic surface of the short terminal helix		HslV	GP			hydrophobic pocket of promoter	NULL		NULL	NULL	NULL	NULL	gw60_cell_103_4_633_s_128	11106733	A hydrophobic surface of  the short terminal helix of HslU binds a hydrophobic pocket of a  neighboring HslV protomer.	bind
39405	1	10602	6	NULL	NULL	0	NULL	HslU	NULL		bind	NULL		hydrophobic surface of the short terminal helix		HslV	NULL			hydrophobic pocket of promoter	NULL		0	NULL	NULL	NULL	gw60_cell_103_4_633_s_128	11106733	A hydrophobic surface of  the short terminal helix of HslU binds a hydrophobic pocket of a  neighboring HslV protomer.	bind
47136	1	10603	5	13	NULL	NULL	NULL	thrombin	GP		bind					FpA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_21_18875_s_189	11901150	A hydrophobic/aromatic residue fills systematically the aryl binding site as documented in the crystal structures of thrombin bound to FpA ( 8,  9) or PAR1 ( 17).	bind
47137	2	10603	5	13	NULL	NULL	NULL	thrombin	GP		bind					PAR1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_21_18875_s_189	11901150	A hydrophobic/aromatic residue fills systematically the aryl binding site as documented in the crystal structures of thrombin bound to FpA ( 8,  9) or PAR1 ( 17).	bind
47138	3	10603	5	13	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_21_18875_s_189	11901150	A hydrophobic/aromatic residue fills systematically the aryl binding site as documented in the crystal structures of thrombin bound to FpA ( 8,  9) or PAR1 ( 17).	bind
47139	4	10603	5	NULL	NULL	0	NULL		NULL		fills	NULL	systematically	hydrophobic/aromatic residue			NULL		aryl binding site		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_21_18875_s_189	11901150	A hydrophobic/aromatic residue fills systematically the aryl binding site as documented in the crystal structures of thrombin bound to FpA ( 8,  9) or PAR1 ( 17).	bind
39406	1	10603	6	NULL	NULL	0	NULL	thrombin	NULL		bind	NULL				FpA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_21_18875_s_189	11901150	A hydrophobic/aromatic residue fills systematically the aryl binding site as documented in the crystal structures of thrombin bound to FpA ( 8,  9) or PAR1 ( 17).	bind
39407	2	10603	6	NULL	NULL	0	NULL	thrombin	NULL		bind	NULL				PAR1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_21_18875_s_189	11901150	A hydrophobic/aromatic residue fills systematically the aryl binding site as documented in the crystal structures of thrombin bound to FpA ( 8,  9) or PAR1 ( 17).	bind
39408	3	10603	6	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_21_18875_s_189	11901150	A hydrophobic/aromatic residue fills systematically the aryl binding site as documented in the crystal structures of thrombin bound to FpA ( 8,  9) or PAR1 ( 17).	bind
39409	4	10603	6	NULL	NULL	0	NULL		NULL		fills	NULL	systematically	hydrophobic/aromatic residue			NULL		aryl binding site		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_21_18875_s_189	11901150	A hydrophobic/aromatic residue fills systematically the aryl binding site as documented in the crystal structures of thrombin bound to FpA ( 8,  9) or PAR1 ( 17).	bind
47140	1	10604	5	13	NULL	NULL	NULL	TF	GP		bind					cell cycle genes	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_21_7988_s_238	16702552	A hypergeometric distribution was used to estimate the statistical significance of the binding specificity of the given TF to the cell cycle genes.	bind
39410	1	10604	6	NULL	NULL	0	NULL	TF	NULL		bind	NULL				cell cycle genes	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_103_21_7988_s_238	16702552	A hypergeometric distribution was used to estimate the statistical significance of the binding specificity of the given TF to the cell cycle genes.	bind
47141	1	10605	5	13	NULL	NULL	NULL	CbbR	GP	binding of	introduces					CBR	NucleicAcid	DNA bend within			NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiolrev_21_2_135_s_284	9348665	A hypersensitive site ( Fig. 4) observed in a DNase I footprint suggested that binding of CbbR introduces a DNA bend within the CBR [ 146].	bind
39412	1	10605	6	10	NULL	0	NULL	CbbR	NULL	binding of	introduces 	NULL				CBR	NULL	DNA bend within			NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiolrev_21_2_135_s_284	9348665	A hypersensitive site ( Fig. 4) observed in a DNase I footprint suggested that binding of CbbR introduces a DNA bend within the CBR [ 146].	bind
47142	1	10606	5	13	NULL	NULL	NULL	titin/connectin	GP		bind					actinin	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-muscle-res-cell-motil_26_6-8_16465475_s_5	16465475	A hypertrophic cardiomyopathy-associated titin/connectin  mutation (Arg740Leu) was found to increase the binding to actinin, while  other dilated cardiomyopathy-associated titin/connectin mutations (Ala743Val  and Val54Met) decreased the binding to actinin and Tcap/telethonin, respectively.	bind
47143	3	10606	5	13	NULL	NULL	NULL	statement 2	Process		increases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-muscle-res-cell-motil_26_6-8_16465475_s_5	16465475	A hypertrophic cardiomyopathy-associated titin/connectin  mutation (Arg740Leu) was found to increase the binding to actinin, while  other dilated cardiomyopathy-associated titin/connectin mutations (Ala743Val  and Val54Met) decreased the binding to actinin and Tcap/telethonin, respectively.	bind
47144	2	10606	5	13	NULL	NULL	NULL	titin/connectin	GP	mutant	is associated with			Arg740Leu		hypertrophic cardiomyopathy	MedicalFinding				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-muscle-res-cell-motil_26_6-8_16465475_s_5	16465475	A hypertrophic cardiomyopathy-associated titin/connectin  mutation (Arg740Leu) was found to increase the binding to actinin, while  other dilated cardiomyopathy-associated titin/connectin mutations (Ala743Val  and Val54Met) decreased the binding to actinin and Tcap/telethonin, respectively.	bind
47145	5	10606	5	13	NULL	NULL	NULL	statement 4	Process		decreases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-muscle-res-cell-motil_26_6-8_16465475_s_5	16465475	A hypertrophic cardiomyopathy-associated titin/connectin  mutation (Arg740Leu) was found to increase the binding to actinin, while  other dilated cardiomyopathy-associated titin/connectin mutations (Ala743Val  and Val54Met) decreased the binding to actinin and Tcap/telethonin, respectively.	bind
47146	4	10606	5	13	NULL	NULL	NULL	titin/connectin	GP	mutant	is associated with			Ala743Val		dilated cardiomyopathy	MedicalFinding				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-muscle-res-cell-motil_26_6-8_16465475_s_5	16465475	A hypertrophic cardiomyopathy-associated titin/connectin  mutation (Arg740Leu) was found to increase the binding to actinin, while  other dilated cardiomyopathy-associated titin/connectin mutations (Ala743Val  and Val54Met) decreased the binding to actinin and Tcap/telethonin, respectively.	bind
47147	6	10606	5	13	NULL	NULL	NULL	titin/connectin	GP	mutant	is associated with			Val54Met		dilated cardiomyopathy	MedicalFinding				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-muscle-res-cell-motil_26_6-8_16465475_s_5	16465475	A hypertrophic cardiomyopathy-associated titin/connectin  mutation (Arg740Leu) was found to increase the binding to actinin, while  other dilated cardiomyopathy-associated titin/connectin mutations (Ala743Val  and Val54Met) decreased the binding to actinin and Tcap/telethonin, respectively.	bind
47148	7	10606	5	13	NULL	NULL	NULL	titin/connectin	GP		bind					Tcap/telethonin	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-muscle-res-cell-motil_26_6-8_16465475_s_5	16465475	A hypertrophic cardiomyopathy-associated titin/connectin  mutation (Arg740Leu) was found to increase the binding to actinin, while  other dilated cardiomyopathy-associated titin/connectin mutations (Ala743Val  and Val54Met) decreased the binding to actinin and Tcap/telethonin, respectively.	bind
57598	8	10606	5	13	NULL	NULL	NULL	statement 6	Process		decreases					statement 7	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-muscle-res-cell-motil_26_6-8_16465475_s_5	16465475	A hypertrophic cardiomyopathy-associated titin/connectin  mutation (Arg740Leu) was found to increase the binding to actinin, while  other dilated cardiomyopathy-associated titin/connectin mutations (Ala743Val  and Val54Met) decreased the binding to actinin and Tcap/telethonin, respectively.	bind
39869	1	10606	6	NULL	NULL	0	NULL	titin/connectin	NULL		bind	NULL				actinin	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-muscle-res-cell-motil_26_6-8_16465475_s_5	16465475	A hypertrophic cardiomyopathy-associated titin/connectin  mutation (Arg740Leu) was found to increase the binding to actinin, while  other dilated cardiomyopathy-associated titin/connectin mutations (Ala743Val  and Val54Met) decreased the binding to actinin and Tcap/telethonin, respectively.	bind
39870	2	10606	6	10	NULL	0	NULL	titin/connectin		mutant	increases			Arg740Leu		statement 1					NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-muscle-res-cell-motil_26_6-8_16465475_s_5	16465475	A hypertrophic cardiomyopathy-associated titin/connectin  mutation (Arg740Leu) was found to increase the binding to actinin, while  other dilated cardiomyopathy-associated titin/connectin mutations (Ala743Val  and Val54Met) decreased the binding to actinin and Tcap/telethonin, respectively.	bind
39871	3	10606	6	10	NULL	0	NULL	titin/connectin		mutant	decreases			Ala743Val		statement 1					NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-muscle-res-cell-motil_26_6-8_16465475_s_5	16465475	A hypertrophic cardiomyopathy-associated titin/connectin  mutation (Arg740Leu) was found to increase the binding to actinin, while  other dilated cardiomyopathy-associated titin/connectin mutations (Ala743Val  and Val54Met) decreased the binding to actinin and Tcap/telethonin, respectively.	bind
39872	4	10606	6	NULL	NULL	0	NULL	titin/connectin	NULL		bind	NULL				Tcap/telethonin	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-muscle-res-cell-motil_26_6-8_16465475_s_5	16465475	A hypertrophic cardiomyopathy-associated titin/connectin  mutation (Arg740Leu) was found to increase the binding to actinin, while  other dilated cardiomyopathy-associated titin/connectin mutations (Ala743Val  and Val54Met) decreased the binding to actinin and Tcap/telethonin, respectively.	bind
39873	5	10606	6	10	NULL	0	NULL	titin/connectin		mutant	decreases			Val54Met		statement 4					NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-muscle-res-cell-motil_26_6-8_16465475_s_5	16465475	A hypertrophic cardiomyopathy-associated titin/connectin  mutation (Arg740Leu) was found to increase the binding to actinin, while  other dilated cardiomyopathy-associated titin/connectin mutations (Ala743Val  and Val54Met) decreased the binding to actinin and Tcap/telethonin, respectively.	bind
40396	6	10606	6	10	NULL	0	NULL	statement 2	NULL		is associated with	NULL				hypertrophic cardiomyopathy	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-muscle-res-cell-motil_26_6-8_16465475_s_5	16465475	A hypertrophic cardiomyopathy-associated titin/connectin  mutation (Arg740Leu) was found to increase the binding to actinin, while  other dilated cardiomyopathy-associated titin/connectin mutations (Ala743Val  and Val54Met) decreased the binding to actinin and Tcap/telethonin, respectively.	bind
40397	7	10606	6	10	NULL	0	NULL	statement 3	NULL		is associated with	NULL				 dilated cardiomyopathy	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-muscle-res-cell-motil_26_6-8_16465475_s_5	16465475	A hypertrophic cardiomyopathy-associated titin/connectin  mutation (Arg740Leu) was found to increase the binding to actinin, while  other dilated cardiomyopathy-associated titin/connectin mutations (Ala743Val  and Val54Met) decreased the binding to actinin and Tcap/telethonin, respectively.	bind
40398	8	10606	6	10	NULL	0	NULL	statement 5	NULL		is associated with	NULL				dilated cardiomyopathy	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-muscle-res-cell-motil_26_6-8_16465475_s_5	16465475	A hypertrophic cardiomyopathy-associated titin/connectin  mutation (Arg740Leu) was found to increase the binding to actinin, while  other dilated cardiomyopathy-associated titin/connectin mutations (Ala743Val  and Val54Met) decreased the binding to actinin and Tcap/telethonin, respectively.	bind
47149	1	10607	5	13	NULL	NULL	NULL	Mks1p	GP	hypophosphorylated;;inactive	bind					Rtg2p	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_mol-cell_12_2_14536080_s_6	14536080	A hypophosphorylated form of Mks1p bound to Rtg2p is inactive.	bind
39415	1	10607	6	10	NULL	0	NULL	Mks1p	NULL	hypophosphorylated;; inactive	bind	NULL				Rtg2p	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_mol-cell_12_2_14536080_s_6	14536080	A hypophosphorylated form of Mks1p bound to Rtg2p is inactive.	bind
47150	1	10608	5	13	NULL	NULL	NULL	DnaA protein	GP		bind		possibly							DnaA boxes	NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_26_4_355_s_548	12413665	A hypothesis has been formulated [   and   ] that postulates that initially all newly synthesized DnaA protein is bound to DnaA  boxes around the chromosome.	bind
47151	2	10608	5	13	NULL	NULL	NULL	statement 1	Process		occurs around		possibly			chromosome	Chromosome				NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_26_4_355_s_548	12413665	A hypothesis has been formulated [   and   ] that postulates that initially all newly synthesized DnaA protein is bound to DnaA  boxes around the chromosome.	bind
39418	1	10608	6	NULL	NULL	0	NULL	DnaA protein	NULL		bind	NULL					NULL			DnaA box	NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_26_4_355_s_548	12413665	A hypothesis has been formulated [   and   ] that postulates that initially all newly synthesized DnaA protein is bound to DnaA  boxes around the chromosome.	bind
39419	2	10608	6	NULL	NULL	0	NULL	statement 1	NULL		occurs around the	NULL				chromosome	NULL				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_26_4_355_s_548	12413665	A hypothesis has been formulated [   and   ] that postulates that initially all newly synthesized DnaA protein is bound to DnaA  boxes around the chromosome.	bind
47154	1	10610	5	13	NULL	NULL	NULL	IGF-I	GP		bind					IGF-I receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_13_8189_s_311	9079636	A hypothetical explanation for this difference is that IGF-I binds to the IGF-I receptor and induces a conformational change by simultaneously bridging the high and low affinity sites ( 42).	bind
47155	2	10610	5	13	NULL	NULL	NULL	statement 1	Process		induces					conformational change	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_13_8189_s_311	9079636	A hypothetical explanation for this difference is that IGF-I binds to the IGF-I receptor and induces a conformational change by simultaneously bridging the high and low affinity sites ( 42).	bind
39422	1	10610	6	NULL	NULL	0	NULL	IGF-I	NULL		bind	NULL				IGF-I receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_13_8189_s_311	9079636	A hypothetical explanation for this difference is that IGF-I binds to the IGF-I receptor and induces a conformational change by simultaneously bridging the high and low affinity sites ( 42).	bind
49999	2	10610	6	10	NULL	0	NULL	statement 1	NULL		induce	NULL				conformational change	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_13_8189_s_311	9079636	A hypothetical explanation for this difference is that IGF-I binds to the IGF-I receptor and induces a conformational change by simultaneously bridging the high and low affinity sites ( 42).	bind
47160	1	10611	5	13	NULL	NULL	NULL	Hfq	GP		bind					rpoS mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_3_373_s_288	12208995	A hypothetical model consistent with all data available would be that Hfq bound to  rpoS mRNA recruits DsrA into a ternary complex (in which secondary structures of  rpoS mRNA and/or of DsrA could also be altered) and thereby facilitate translational stimulation by DsrA.	bind
47161	2	10611	5	13	NULL	NULL	NULL	DsrA	GP		is recruited to					ternary complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_3_373_s_288	12208995	A hypothetical model consistent with all data available would be that Hfq bound to  rpoS mRNA recruits DsrA into a ternary complex (in which secondary structures of  rpoS mRNA and/or of DsrA could also be altered) and thereby facilitate translational stimulation by DsrA.	bind
47162	3	10611	5	13	NULL	NULL	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_3_373_s_288	12208995	A hypothetical model consistent with all data available would be that Hfq bound to  rpoS mRNA recruits DsrA into a ternary complex (in which secondary structures of  rpoS mRNA and/or of DsrA could also be altered) and thereby facilitate translational stimulation by DsrA.	bind
47163	4	10611	5	13	NULL	NULL	NULL	statement 2	Process		alters		may			rpoS mRNA	NucleicAcid	secondary structure of			NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_3_373_s_288	12208995	A hypothetical model consistent with all data available would be that Hfq bound to  rpoS mRNA recruits DsrA into a ternary complex (in which secondary structures of  rpoS mRNA and/or of DsrA could also be altered) and thereby facilitate translational stimulation by DsrA.	bind
47164	5	10611	5	13	NULL	NULL	NULL	statement 2	Process		alters		may			DsrA	GP	secondary structure of			NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_3_373_s_288	12208995	A hypothetical model consistent with all data available would be that Hfq bound to  rpoS mRNA recruits DsrA into a ternary complex (in which secondary structures of  rpoS mRNA and/or of DsrA could also be altered) and thereby facilitate translational stimulation by DsrA.	bind
47165	6	10611	5	13	NULL	NULL	NULL	DsrA	GP		carries out					translational stimulation	Process				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_3_373_s_288	12208995	A hypothetical model consistent with all data available would be that Hfq bound to  rpoS mRNA recruits DsrA into a ternary complex (in which secondary structures of  rpoS mRNA and/or of DsrA could also be altered) and thereby facilitate translational stimulation by DsrA.	bind
47166	7	10611	5	13	NULL	NULL	NULL	statement 3	Process		facilitates		potentially			statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_3_373_s_288	12208995	A hypothetical model consistent with all data available would be that Hfq bound to  rpoS mRNA recruits DsrA into a ternary complex (in which secondary structures of  rpoS mRNA and/or of DsrA could also be altered) and thereby facilitate translational stimulation by DsrA.	bind
39423	1	10611	6	NULL	NULL	0	NULL	Hfq	NULL		bind	NULL				rpoS mRNA	NULL				NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_3_373_s_288	12208995	A hypothetical model consistent with all data available would be that Hfq bound to  rpoS mRNA recruits DsrA into a ternary complex (in which secondary structures of  rpoS mRNA and/or of DsrA could also be altered) and thereby facilitate translational stimulation by DsrA.	bind
39424	2	10611	6	NULL	NULL	0	NULL	statement 1	NULL		recruits	NULL				DsrA	NULL				NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_3_373_s_288	12208995	A hypothetical model consistent with all data available would be that Hfq bound to  rpoS mRNA recruits DsrA into a ternary complex (in which secondary structures of  rpoS mRNA and/or of DsrA could also be altered) and thereby facilitate translational stimulation by DsrA.	bind
39426	3	10611	6	NULL	NULL	0	NULL	DsrA	NULL		is recruited into	NULL				ternary complex	NULL				NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_3_373_s_288	12208995	A hypothetical model consistent with all data available would be that Hfq bound to  rpoS mRNA recruits DsrA into a ternary complex (in which secondary structures of  rpoS mRNA and/or of DsrA could also be altered) and thereby facilitate translational stimulation by DsrA.	bind
39428	4	10611	6	NULL	NULL	0	NULL	DsrA	NULL		carries out	NULL				translational stimulation	NULL				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_3_373_s_288	12208995	A hypothetical model consistent with all data available would be that Hfq bound to  rpoS mRNA recruits DsrA into a ternary complex (in which secondary structures of  rpoS mRNA and/or of DsrA could also be altered) and thereby facilitate translational stimulation by DsrA.	bind
39430	5	10611	6	NULL	NULL	0	NULL	statement 2	NULL		facilitates	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_3_373_s_288	12208995	A hypothetical model consistent with all data available would be that Hfq bound to  rpoS mRNA recruits DsrA into a ternary complex (in which secondary structures of  rpoS mRNA and/or of DsrA could also be altered) and thereby facilitate translational stimulation by DsrA.	bind
39432	6	10611	6	NULL	NULL	0	NULL	statement 2	NULL		alters	NULL	could			rpoS mRNA	NULL	secondary structure of 			NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_3_373_s_288	12208995	A hypothetical model consistent with all data available would be that Hfq bound to  rpoS mRNA recruits DsrA into a ternary complex (in which secondary structures of  rpoS mRNA and/or of DsrA could also be altered) and thereby facilitate translational stimulation by DsrA.	bind
39434	7	10611	6	NULL	NULL	0	NULL	statement 2	NULL		alters	NULL	could			DsrA	NULL	secondary structure of			NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_66_3_373_s_288	12208995	A hypothetical model consistent with all data available would be that Hfq bound to  rpoS mRNA recruits DsrA into a ternary complex (in which secondary structures of  rpoS mRNA and/or of DsrA could also be altered) and thereby facilitate translational stimulation by DsrA.	bind
47167	3	10612	5	13	NULL	NULL	NULL	statement 1	Process		influences		possibly			integrin affinity	Process	modulation of			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_6_1799_s_286	10359597	A hypothetical scheme of how the GTP-binding cycles of Ras and R-Ras could influence integrin affinity modulation.	bind
47168	4	10612	5	13	NULL	NULL	NULL	statement 2	Process		influences		possibly			integrin affinity	Process	modulation of			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_6_1799_s_286	10359597	A hypothetical scheme of how the GTP-binding cycles of Ras and R-Ras could influence integrin affinity modulation.	bind
50000	1	10612	5	13	NULL	NULL	NULL	Ras	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_6_1799_s_286	10359597	A hypothetical scheme of how the GTP-binding cycles of Ras and R-Ras could influence integrin affinity modulation.	bind
50001	2	10612	5	13	NULL	NULL	NULL	R-Ras	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_6_1799_s_286	10359597	A hypothetical scheme of how the GTP-binding cycles of Ras and R-Ras could influence integrin affinity modulation.	bind
39470	1	10612	6	NULL	NULL	0	NULL	Ras	NULL		bind	NULL				GTP	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_10_6_1799_s_286	10359597	A hypothetical scheme of how the GTP-binding cycles of Ras and R-Ras could influence integrin affinity modulation.	bind
39471	2	10612	6	NULL	NULL	0	NULL	R-Ras	NULL		bind	NULL				GTP	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_10_6_1799_s_286	10359597	A hypothetical scheme of how the GTP-binding cycles of Ras and R-Ras could influence integrin affinity modulation.	bind
39472	3	10612	6	NULL	NULL	0	NULL	statement 1	NULL		influence	NULL	may			integrin affinity	NULL	modulation of 			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_10_6_1799_s_286	10359597	A hypothetical scheme of how the GTP-binding cycles of Ras and R-Ras could influence integrin affinity modulation.	bind
39473	4	10612	6	NULL	NULL	0	NULL	statement 2	NULL		influence	NULL	may			integrin affinity	NULL	modulation of			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_10_6_1799_s_286	10359597	A hypothetical scheme of how the GTP-binding cycles of Ras and R-Ras could influence integrin affinity modulation.	bind
47169	1	10613	5	13	NULL	NULL	NULL	hypoxia-inducible factor	GP		bind					VEGF	GP			enhancer	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_77_3_638_s_127	7641334	A hypoxia-inducible factor binds to the VEGF enhancer.	bind
39474	1	10613	6	NULL	NULL	0	NULL	hypoxia-inducible factor	NULL		bind	NULL				VEGF	NULL			enhancer	NULL		0	NULL	NULL	NULL	gw60_circulationres_77_3_638_s_127	7641334	A hypoxia-inducible factor binds to the VEGF enhancer.	bind
47170	1	10615	5	13	NULL	NULL	NULL	transcription factor	GP		bind							sequences resembling		interferon- activation site	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_966_s_142	7822337	A Jak-type kinase  probably mediates IL-4-stimulated tyrosine phosphorylation of a  transcription factor that binds to sequences resembling the  interferon-   activation site and increases transcriptional activity  in reporter gene assays( 46 ,  47 ,  48 ) .	bind
47171	2	10615	5	13	NULL	NULL	NULL	statement 1	GP		increases					transcriptional activity	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_966_s_142	7822337	A Jak-type kinase  probably mediates IL-4-stimulated tyrosine phosphorylation of a  transcription factor that binds to sequences resembling the  interferon-   activation site and increases transcriptional activity  in reporter gene assays( 46 ,  47 ,  48 ) .	bind
47172	3	10615	5	13	NULL	NULL	NULL	IL-4	GP		stimulate					statement 1	Process	phosphorylation of	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_966_s_142	7822337	A Jak-type kinase  probably mediates IL-4-stimulated tyrosine phosphorylation of a  transcription factor that binds to sequences resembling the  interferon-   activation site and increases transcriptional activity  in reporter gene assays( 46 ,  47 ,  48 ) .	bind
47173	4	10615	5	13	NULL	NULL	NULL	Jak-type kinase	GP		mediates		probably			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_966_s_142	7822337	A Jak-type kinase  probably mediates IL-4-stimulated tyrosine phosphorylation of a  transcription factor that binds to sequences resembling the  interferon-   activation site and increases transcriptional activity  in reporter gene assays( 46 ,  47 ,  48 ) .	bind
50758	1	10615	6	10	NULL	0	NULL	transcription factor	NULL		bind	NULL					NULL	sequence resembling		interferon- activation site	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_2_966_s_142	7822337	A Jak-type kinase  probably mediates IL-4-stimulated tyrosine phosphorylation of a  transcription factor that binds to sequences resembling the  interferon-   activation site and increases transcriptional activity  in reporter gene assays( 46 ,  47 ,  48 ) .	bind
50759	2	10615	6	10	NULL	0	NULL	IL-4	NULL		stimulates	NULL				transcription factor	NULL	phosphorylation of	Tyrosine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_2_966_s_142	7822337	A Jak-type kinase  probably mediates IL-4-stimulated tyrosine phosphorylation of a  transcription factor that binds to sequences resembling the  interferon-   activation site and increases transcriptional activity  in reporter gene assays( 46 ,  47 ,  48 ) .	bind
50760	3	10615	6	10	NULL	0	NULL	Jak-type kinase	NULL		mediates	NULL	probably			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_2_966_s_142	7822337	A Jak-type kinase  probably mediates IL-4-stimulated tyrosine phosphorylation of a  transcription factor that binds to sequences resembling the  interferon-   activation site and increases transcriptional activity  in reporter gene assays( 46 ,  47 ,  48 ) .	bind
47205	1	10616	5	13	NULL	NULL	NULL	DNS-SsrA peptide	GP		bind					ClpA hexamer	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_13_12221_s_181	15657062	A Job plot based on the method of continuous variations ( ) of DNS-SsrA peptide binding to ClpA6 shows a maximum at a molar ratio of protein to peptide of 0.45, indicating that approximately 1 mol of DNS-SsrA peptide binds to the 1 mol of ClpA hexamer ( Fig. 5 A).	bind
39475	1	10616	6	NULL	NULL	0	NULL	DNS-SsrA peptide	NULL		bind	NULL				ClpA hexamer	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_13_12221_s_181	15657062	A Job plot based on the method of continuous variations ( ) of DNS-SsrA peptide binding to ClpA6 shows a maximum at a molar ratio of protein to peptide of 0.45, indicating that approximately 1 mol of DNS-SsrA peptide binds to the 1 mol of ClpA hexamer ( Fig. 5 A).	bind
47206	1	10617	5	13	NULL	NULL	NULL	NAD+	Chemical		bind					IPS	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_12_11475_s_53	15653679	A Jobin y Van Fluoromax 3 spectrofluorimeter was used to monitor the binding of NAD+ to IPS and IPS mutants ( 1 muM in 10 mM EDTA with 10 mM KH2PO4, pH 7).	bind
47207	2	10617	5	13	NULL	NULL	NULL	NAD+	Chemical		bind					IPS	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_12_11475_s_53	15653679	A Jobin y Van Fluoromax 3 spectrofluorimeter was used to monitor the binding of NAD+ to IPS and IPS mutants ( 1 muM in 10 mM EDTA with 10 mM KH2PO4, pH 7).	bind
39515	1	10617	6	NULL	NULL	0	NULL	NAD+	NULL		bind	NULL				IPS	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_12_11475_s_53	15653679	A Jobin y Van Fluoromax 3 spectrofluorimeter was used to monitor the binding of NAD+ to IPS and IPS mutants ( 1 muM in 10 mM EDTA with 10 mM KH2PO4, pH 7).	bind
39516	2	10617	6	NULL	NULL	0	NULL	NAD+	NULL		bind	NULL				IPS	NULL	mutant			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_12_11475_s_53	15653679	A Jobin y Van Fluoromax 3 spectrofluorimeter was used to monitor the binding of NAD+ to IPS and IPS mutants ( 1 muM in 10 mM EDTA with 10 mM KH2PO4, pH 7).	bind
47208	1	10618	5	13	NULL	NULL	NULL	insulin receptor	GP	mutant	lacks			K1018A		tyrosine kinase activity					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15985_s_207	10821852	A K1018A mutant of the insulin receptor lacking tyrosine kinase activity does not bind to SOCS-3 (row 2).	bind
47209	2	10618	5	13	NULL	NULL	NULL	insulin receptor	GP	mutant	does not bind			K1018A		SOCS-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15985_s_207	10821852	A K1018A mutant of the insulin receptor lacking tyrosine kinase activity does not bind to SOCS-3 (row 2).	bind
39517	1	10618	6	NULL	NULL	0	NULL	insulin receptor	NULL	mutant	lacks	NULL		K1018A		tyrosine kinase activity	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15985_s_207	10821852	A K1018A mutant of the insulin receptor lacking tyrosine kinase activity does not bind to SOCS-3 (row 2).	bind
39518	2	10618	6	10	NULL	0	NULL	insulin receptor		mutant	does not bind			K1018A		SOCS-3					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15985_s_207	10821852	A K1018A mutant of the insulin receptor lacking tyrosine kinase activity does not bind to SOCS-3 (row 2).	bind
47210	1	10619	5	13	NULL	NULL	NULL				is substituted in			K215R		Isw2p	GP	putative	ATP-binding pocket		NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_8_942_s_106	15833917	A K215R substitution in the putative ATP-binding pocket of Isw2p reduces ATPase activity to background levels without affecting Isw2 complex integrity (Gelbart et al. 2001 ; Fitzgerald et al. 2004 ).	bind
47211	2	10619	5	13	NULL	NULL	NULL	statement 1	Process		reduces					ATPase 	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_8_942_s_106	15833917	A K215R substitution in the putative ATP-binding pocket of Isw2p reduces ATPase activity to background levels without affecting Isw2 complex integrity (Gelbart et al. 2001 ; Fitzgerald et al. 2004 ).	bind
47212	3	10619	5	13	NULL	NULL	NULL	statement 2	Process		does not affect					Isw2 complex	GP	integrity of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_8_942_s_106	15833917	A K215R substitution in the putative ATP-binding pocket of Isw2p reduces ATPase activity to background levels without affecting Isw2 complex integrity (Gelbart et al. 2001 ; Fitzgerald et al. 2004 ).	bind
39874	1	10619	6	10	NULL	0	NULL	Isw2p		mutant;; putative	reduces			K215R ;; ATP-binding pocket		ATPase 		activity of 			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_8_942_s_106	15833917	A K215R substitution in the putative ATP-binding pocket of Isw2p reduces ATPase activity to background levels without affecting Isw2 complex integrity (Gelbart et al. 2001 ; Fitzgerald et al. 2004 ).	bind
39875	2	10619	6	NULL	NULL	0	NULL	Isw2p	NULL	mutant;; putative	does not affect	NULL		K215R ;; ATP-binding pocket		Isw2 complex	NULL	integrity of			NULL		0	NULL	NULL	NULL	gw70_genesdev_19_8_942_s_106	15833917	A K215R substitution in the putative ATP-binding pocket of Isw2p reduces ATPase activity to background levels without affecting Isw2 complex integrity (Gelbart et al. 2001 ; Fitzgerald et al. 2004 ).	bind
47213	1	10620	5	13	NULL	NULL	NULL	XPD	GP	canonical	is mutated in			GKS/T ATP binding motif					K48R		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_21_7355_s_27	11585917	A K48R mutation in the canonical GKS/T ATP binding motif of XPD or the Rad3 homolog abolishes repair but does not compromise transcription ( 43,  66).	bind
47214	2	10620	5	13	NULL	NULL	NULL	statement 1	Process		abolishes					repair	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_21_7355_s_27	11585917	A K48R mutation in the canonical GKS/T ATP binding motif of XPD or the Rad3 homolog abolishes repair but does not compromise transcription ( 43,  66).	bind
47215	3	10620	5	13	NULL	NULL	NULL	statement 1	Process		does not compromise					transcription	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_21_7355_s_27	11585917	A K48R mutation in the canonical GKS/T ATP binding motif of XPD or the Rad3 homolog abolishes repair but does not compromise transcription ( 43,  66).	bind
47216	4	10620	5	13	NULL	NULL	NULL	Rad3 homolog	GP	canonical	is mutated in			GKS/T ATP binding motif					K48R		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_21_7355_s_27	11585917	A K48R mutation in the canonical GKS/T ATP binding motif of XPD or the Rad3 homolog abolishes repair but does not compromise transcription ( 43,  66).	bind
47217	5	10620	5	13	NULL	NULL	NULL	statement 4	Process		abolishes					repair	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_21_7355_s_27	11585917	A K48R mutation in the canonical GKS/T ATP binding motif of XPD or the Rad3 homolog abolishes repair but does not compromise transcription ( 43,  66).	bind
47218	6	10620	5	13	NULL	NULL	NULL	statement 4	Process		does not compromise					transcription	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_21_7355_s_27	11585917	A K48R mutation in the canonical GKS/T ATP binding motif of XPD or the Rad3 homolog abolishes repair but does not compromise transcription ( 43,  66).	bind
39876	1	10620	6	NULL	NULL	0	NULL	XPD	NULL	mutant	abolishes	NULL		K48R;; GKS/T ATP binding motif		repair	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_21_7355_s_27	11585917	A K48R mutation in the canonical GKS/T ATP binding motif of XPD or the Rad3 homolog abolishes repair but does not compromise transcription ( 43,  66).	bind
39877	2	10620	6	NULL	NULL	0	NULL	rad3 homolog	NULL	mutant	abolishes	NULL		K48R;; GKS/T ATP binding motif		repair	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_21_7355_s_27	11585917	A K48R mutation in the canonical GKS/T ATP binding motif of XPD or the Rad3 homolog abolishes repair but does not compromise transcription ( 43,  66).	bind
39878	3	10620	6	NULL	NULL	0	NULL	XPD	NULL	mutant	has no effect on	NULL		K48R;; GKS/T ATP binding motif		transcription	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_21_7355_s_27	11585917	A K48R mutation in the canonical GKS/T ATP binding motif of XPD or the Rad3 homolog abolishes repair but does not compromise transcription ( 43,  66).	bind
39879	4	10620	6	NULL	NULL	0	NULL	rad3 homolog	NULL	mutant	has no effect on	NULL		K48R;; GKS/T ATP binding motif		transcription	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_21_7355_s_27	11585917	A K48R mutation in the canonical GKS/T ATP binding motif of XPD or the Rad3 homolog abolishes repair but does not compromise transcription ( 43,  66).	bind
47220	1	10621	5	13	NULL	NULL	NULL	serine proteinase/serpin complex	GP		bind					very-low-density lipoprotein receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_atherosclerosis_141_2_191_s_493	9862168	A Kasza, HH Petersen, CW Heegaard, K Oka, A Christensen, A Dubin, L Chan and PA. Andreasen, Specificity of serine proteinase/serpin complex binding to very-low-density lipoprotein receptor and  2-macroglobulin receptor/low-density-lipoprotein-receptor-related protein.	bind
47223	2	10621	5	13	NULL	NULL	NULL	serine proteinase/serpin complex	GP		bind					2-macroglobulin receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_atherosclerosis_141_2_191_s_493	9862168	A Kasza, HH Petersen, CW Heegaard, K Oka, A Christensen, A Dubin, L Chan and PA. Andreasen, Specificity of serine proteinase/serpin complex binding to very-low-density lipoprotein receptor and  2-macroglobulin receptor/low-density-lipoprotein-receptor-related protein.	bind
47224	3	10621	5	13	NULL	NULL	NULL	2-macroglobulin receptor	GP		is a type of					low-density-lipoprotein-receptor-related protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_atherosclerosis_141_2_191_s_493	9862168	A Kasza, HH Petersen, CW Heegaard, K Oka, A Christensen, A Dubin, L Chan and PA. Andreasen, Specificity of serine proteinase/serpin complex binding to very-low-density lipoprotein receptor and  2-macroglobulin receptor/low-density-lipoprotein-receptor-related protein.	bind
39519	1	10621	6	NULL	NULL	0	NULL	serine proteinase/serpin complex	NULL		bind	NULL				very-low-density lipoprotein receptor 	NULL				NULL		0	NULL	NULL	NULL	gw60_atherosclerosis_141_2_191_s_493	9862168	A Kasza, HH Petersen, CW Heegaard, K Oka, A Christensen, A Dubin, L Chan and PA. Andreasen, Specificity of serine proteinase/serpin complex binding to very-low-density lipoprotein receptor and  2-macroglobulin receptor/low-density-lipoprotein-receptor-related protein.	bind
39520	2	10621	6	NULL	NULL	0	NULL	serine proteinase/serpin complex	NULL		bind	NULL				2-macroglobulin receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_atherosclerosis_141_2_191_s_493	9862168	A Kasza, HH Petersen, CW Heegaard, K Oka, A Christensen, A Dubin, L Chan and PA. Andreasen, Specificity of serine proteinase/serpin complex binding to very-low-density lipoprotein receptor and  2-macroglobulin receptor/low-density-lipoprotein-receptor-related protein.	bind
39521	3	10621	6	NULL	NULL	0	NULL	2-macroglobulin receptor	NULL		is a type of	NULL				low-density-lipoprotein-receptor-related protein	NULL				NULL		0	NULL	NULL	NULL	gw60_atherosclerosis_141_2_191_s_493	9862168	A Kasza, HH Petersen, CW Heegaard, K Oka, A Christensen, A Dubin, L Chan and PA. Andreasen, Specificity of serine proteinase/serpin complex binding to very-low-density lipoprotein receptor and  2-macroglobulin receptor/low-density-lipoprotein-receptor-related protein.	bind
47225	1	10622	5	13	NULL	NULL	NULL	KEP1 protein	GP	truncated	bind			GSG domain		poly(U) homopolymeric RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_46_30122_s_185	9804767	A KEP1 truncation protein encompassing the entire GSG domain bound poly(U) homopolymeric RNA (Fig.  5 A, KEP:1-224).	bind
39522	1	10622	6	NULL	NULL	0	NULL	KEP1 protein	NULL	truncated	bind	NULL		GSG domain		poly(U) homopolymeric RNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_46_30122_s_185	9804767	A KEP1 truncation protein encompassing the entire GSG domain bound poly(U) homopolymeric RNA (Fig.  5 A, KEP:1-224).	bind
47227	1	10623	5	13	NULL	NULL	NULL	ketoconazole molecule	Chemical		bind			imidazole nitrogen		heme iron	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_37_13682_s_63	16954191	A ketoconazole molecule with its imidazole nitrogen bound to the heme iron could unambiguously be modeled into electron density in all four molecules in the asymmetric unit ( Fig. 3).	bind
39557	1	10623	6	NULL	NULL	0	NULL	ketoconazole molecule	NULL		bind	NULL		imidazole nitrogen		heme iron	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_103_37_13682_s_63	16954191	A ketoconazole molecule with its imidazole nitrogen bound to the heme iron could unambiguously be modeled into electron density in all four molecules in the asymmetric unit ( Fig. 3).	bind
47228	1	10624	5	13	NULL	NULL	NULL	Vps10p	GP		is a type of					type I transmembrane receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_10_3242_s_21	11598206	A key component in the sorting and transport of vacuolar hydrolases is Vps10p, a type I transmembrane receptor that binds vacuolar hydrolases in the late-Golgi (Marcusson  et al., 1994  ; Cooper and Stevens, 1996  ).	bind
47229	2	10624	5	13	NULL	NULL	NULL	Vps10p	GP		bind					vacuolar hydrolases	GP				NULL	late-Golgi	NULL	NULL	NULL	NULL	gw60_molbiolcell_12_10_3242_s_21	11598206	A key component in the sorting and transport of vacuolar hydrolases is Vps10p, a type I transmembrane receptor that binds vacuolar hydrolases in the late-Golgi (Marcusson  et al., 1994  ; Cooper and Stevens, 1996  ).	bind
47230	3	10624	5	13	NULL	NULL	NULL	Vps10p	GP		plays a role in					vacuolar hydrolases	GP	sorting of			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_10_3242_s_21	11598206	A key component in the sorting and transport of vacuolar hydrolases is Vps10p, a type I transmembrane receptor that binds vacuolar hydrolases in the late-Golgi (Marcusson  et al., 1994  ; Cooper and Stevens, 1996  ).	bind
47232	4	10624	5	13	NULL	NULL	NULL	Vps10p	GP		plays a role in					vacuolar hydrolases	GP	transport of			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_10_3242_s_21	11598206	A key component in the sorting and transport of vacuolar hydrolases is Vps10p, a type I transmembrane receptor that binds vacuolar hydrolases in the late-Golgi (Marcusson  et al., 1994  ; Cooper and Stevens, 1996  ).	bind
39558	1	10624	6	NULL	NULL	0	NULL	Vps10p	NULL		is a type of	NULL				type I transmembrane receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_10_3242_s_21	11598206	A key component in the sorting and transport of vacuolar hydrolases is Vps10p, a type I transmembrane receptor that binds vacuolar hydrolases in the late-Golgi (Marcusson  et al., 1994  ; Cooper and Stevens, 1996  ).	bind
39559	2	10624	6	NULL	NULL	0	NULL	Vps10p	NULL		bind	NULL				vacuolar hydrolases	NULL				NULL	late golgi	0	NULL	NULL	NULL	gw60_molbiolcell_12_10_3242_s_21	11598206	A key component in the sorting and transport of vacuolar hydrolases is Vps10p, a type I transmembrane receptor that binds vacuolar hydrolases in the late-Golgi (Marcusson  et al., 1994  ; Cooper and Stevens, 1996  ).	bind
39560	3	10624	6	NULL	NULL	0	NULL	Vps10p	NULL		plays a role in	NULL				vacuolar hydrolases	NULL	sorting of			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_10_3242_s_21	11598206	A key component in the sorting and transport of vacuolar hydrolases is Vps10p, a type I transmembrane receptor that binds vacuolar hydrolases in the late-Golgi (Marcusson  et al., 1994  ; Cooper and Stevens, 1996  ).	bind
39561	4	10624	6	NULL	NULL	0	NULL	Vps10p	NULL		plays a role in	NULL				vacuolar hydrolases	NULL	transport of 			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_10_3242_s_21	11598206	A key component in the sorting and transport of vacuolar hydrolases is Vps10p, a type I transmembrane receptor that binds vacuolar hydrolases in the late-Golgi (Marcusson  et al., 1994  ; Cooper and Stevens, 1996  ).	bind
47233	1	10625	5	13	NULL	NULL	NULL	FRS2	GP		plays a role in					FGF signaling	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_3_1747_s_23	14593093	A key component of FGF signaling is the docking protein FRS2, which binds to the FGFRs and recruits several signal transducing molecules leading to the activation of the mitogen-activated protein kinase (MAPK) cascade and the PI3K-AKT antiapoptotic pathway (  -  ).	bind
47234	2	10625	5	13	NULL	NULL	NULL	FRS2	GP		bind					FGFRs	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_3_1747_s_23	14593093	A key component of FGF signaling is the docking protein FRS2, which binds to the FGFRs and recruits several signal transducing molecules leading to the activation of the mitogen-activated protein kinase (MAPK) cascade and the PI3K-AKT antiapoptotic pathway (  -  ).	bind
47235	3	10625	5	13	NULL	NULL	NULL	statement 2	GP		recruits					signal transducing molecules	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_3_1747_s_23	14593093	A key component of FGF signaling is the docking protein FRS2, which binds to the FGFRs and recruits several signal transducing molecules leading to the activation of the mitogen-activated protein kinase (MAPK) cascade and the PI3K-AKT antiapoptotic pathway (  -  ).	bind
47236	4	10625	5	13	NULL	NULL	NULL	statement 3	GP		leads to					MAPK cascade	Process	activation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_3_1747_s_23	14593093	A key component of FGF signaling is the docking protein FRS2, which binds to the FGFRs and recruits several signal transducing molecules leading to the activation of the mitogen-activated protein kinase (MAPK) cascade and the PI3K-AKT antiapoptotic pathway (  -  ).	bind
47239	5	10625	5	13	NULL	NULL	NULL	MAPK	GP		is					mitogen-activated protein kinase	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_3_1747_s_23	14593093	A key component of FGF signaling is the docking protein FRS2, which binds to the FGFRs and recruits several signal transducing molecules leading to the activation of the mitogen-activated protein kinase (MAPK) cascade and the PI3K-AKT antiapoptotic pathway (  -  ).	bind
47241	6	10625	5	13	NULL	NULL	NULL	statement 3	Process		leads to					PI3K-AKT antiapoptotic pathway	Process	activation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_3_1747_s_23	14593093	A key component of FGF signaling is the docking protein FRS2, which binds to the FGFRs and recruits several signal transducing molecules leading to the activation of the mitogen-activated protein kinase (MAPK) cascade and the PI3K-AKT antiapoptotic pathway (  -  ).	bind
47242	7	10625	5	13	NULL	NULL	NULL	FRS2	GP		is a type of					docking protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_3_1747_s_23	14593093	A key component of FGF signaling is the docking protein FRS2, which binds to the FGFRs and recruits several signal transducing molecules leading to the activation of the mitogen-activated protein kinase (MAPK) cascade and the PI3K-AKT antiapoptotic pathway (  -  ).	bind
39562	1	10625	6	NULL	NULL	0	NULL	FRS2	NULL		is a type of	NULL				docking protein	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_3_1747_s_23	14593093	A key component of FGF signaling is the docking protein FRS2, which binds to the FGFRs and recruits several signal transducing molecules leading to the activation of the mitogen-activated protein kinase (MAPK) cascade and the PI3K-AKT antiapoptotic pathway (  -  ).	bind
39563	2	10625	6	NULL	NULL	0	NULL	FRS2	NULL		bind	NULL				FGFR	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_3_1747_s_23	14593093	A key component of FGF signaling is the docking protein FRS2, which binds to the FGFRs and recruits several signal transducing molecules leading to the activation of the mitogen-activated protein kinase (MAPK) cascade and the PI3K-AKT antiapoptotic pathway (  -  ).	bind
39564	3	10625	6	NULL	NULL	0	NULL	FRS2	NULL		is a key component of	NULL				FGF signaling	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_3_1747_s_23	14593093	A key component of FGF signaling is the docking protein FRS2, which binds to the FGFRs and recruits several signal transducing molecules leading to the activation of the mitogen-activated protein kinase (MAPK) cascade and the PI3K-AKT antiapoptotic pathway (  -  ).	bind
39565	4	10625	6	NULL	NULL	0	NULL	statement 2	NULL		recruits	NULL				signal transducing molecules	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_3_1747_s_23	14593093	A key component of FGF signaling is the docking protein FRS2, which binds to the FGFRs and recruits several signal transducing molecules leading to the activation of the mitogen-activated protein kinase (MAPK) cascade and the PI3K-AKT antiapoptotic pathway (  -  ).	bind
39566	5	10625	6	NULL	NULL	0	NULL	statement 4	NULL		leads to	NULL				MAPK cascade	NULL	activation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_3_1747_s_23	14593093	A key component of FGF signaling is the docking protein FRS2, which binds to the FGFRs and recruits several signal transducing molecules leading to the activation of the mitogen-activated protein kinase (MAPK) cascade and the PI3K-AKT antiapoptotic pathway (  -  ).	bind
39567	6	10625	6	NULL	NULL	0	NULL	MAPK	NULL		is	NULL				mitogen-activated protein kinase	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_3_1747_s_23	14593093	A key component of FGF signaling is the docking protein FRS2, which binds to the FGFRs and recruits several signal transducing molecules leading to the activation of the mitogen-activated protein kinase (MAPK) cascade and the PI3K-AKT antiapoptotic pathway (  -  ).	bind
39568	7	10625	6	NULL	NULL	0	NULL	statement 4	NULL		leads to	NULL				PI3K-AKT antiapoptotic pathway	NULL	activation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_3_1747_s_23	14593093	A key component of FGF signaling is the docking protein FRS2, which binds to the FGFRs and recruits several signal transducing molecules leading to the activation of the mitogen-activated protein kinase (MAPK) cascade and the PI3K-AKT antiapoptotic pathway (  -  ).	bind
47246	1	10626	5	13	NULL	NULL	NULL	SH2 domain	GP		is					Src homology 2 domain	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_19_11962_s_23	9565625	A key component of several signaling intermediates is the Src homology 2 (SH2) domain that binds tyrosine-phosphorylated proteins in a sequence-specific manner ( 12).	bind
47247	2	10626	5	13	NULL	NULL	NULL				bind		sequence specifically	SH2 domain		proteins	GP	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_19_11962_s_23	9565625	A key component of several signaling intermediates is the Src homology 2 (SH2) domain that binds tyrosine-phosphorylated proteins in a sequence-specific manner ( 12).	bind
39569	1	10626	6	NULL	NULL	0	NULL		NULL		bind	NULL	sequence specifically	SH2 domain		protein	NULL	phosphorylated	tyrosine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_19_11962_s_23	9565625	A key component of several signaling intermediates is the Src homology 2 (SH2) domain that binds tyrosine-phosphorylated proteins in a sequence-specific manner ( 12).	bind
39570	2	10626	6	NULL	NULL	0	NULL	SH2	NULL		is	NULL				Src homology 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_19_11962_s_23	9565625	A key component of several signaling intermediates is the Src homology 2 (SH2) domain that binds tyrosine-phosphorylated proteins in a sequence-specific manner ( 12).	bind
47248	1	10627	5	13	NULL	NULL	NULL	CD154	GP		is a type of					T-cell - expressed CD40 ligand	GP				NULL		NULL	NULL	NULL	NULL	gw70_diabetes_55_1_27_s_10	16380473	A key costimulatory pathway involves the binding of the T-cell - expressed CD40 ligand (CD154) to CD40 on antigen-presenting cells ( ).	bind
47249	2	10627	5	13	NULL	NULL	NULL	CD154	GP		bind					CD40	GP				NULL	antigen-presenting cells	NULL	NULL	NULL	NULL	gw70_diabetes_55_1_27_s_10	16380473	A key costimulatory pathway involves the binding of the T-cell - expressed CD40 ligand (CD154) to CD40 on antigen-presenting cells ( ).	bind
50002	3	10627	5	13	NULL	NULL	NULL	costimulatory pathway	Process		involves					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_diabetes_55_1_27_s_10	16380473	A key costimulatory pathway involves the binding of the T-cell - expressed CD40 ligand (CD154) to CD40 on antigen-presenting cells ( ).	bind
39571	1	10627	6	10	NULL	0	NULL	CD154	NULL		is a type of	NULL				T-cell-expressed CD40 ligand	NULL				NULL		NULL	NULL	NULL	NULL	gw70_diabetes_55_1_27_s_10	16380473	A key costimulatory pathway involves the binding of the T-cell - expressed CD40 ligand (CD154) to CD40 on antigen-presenting cells ( ).	bind
39572	2	10627	6	NULL	NULL	0	NULL	CD154	NULL		bind	NULL				CD40	NULL				NULL	antigen presenting cells	0	NULL	NULL	NULL	gw70_diabetes_55_1_27_s_10	16380473	A key costimulatory pathway involves the binding of the T-cell - expressed CD40 ligand (CD154) to CD40 on antigen-presenting cells ( ).	bind
39573	3	10627	6	10	NULL	0	NULL	costimulatory pathway	NULL		involves	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_diabetes_55_1_27_s_10	16380473	A key costimulatory pathway involves the binding of the T-cell - expressed CD40 ligand (CD154) to CD40 on antigen-presenting cells ( ).	bind
47252	1	10629	5	13	NULL	NULL	NULL	PDZ proteins	GP		bind					ct-GluR2/3	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_28_3_873_s_247	11163273	A key feature of our model is that the binding of PDZ proteins to ct-GluR2/3 regulates the insertion of receptors.	bind
47253	2	10629	5	13	NULL	NULL	NULL	statement 1	Process		regulates					receptors	GP	insertion of			NULL		NULL	NULL	NULL	NULL	gw60_neuron_28_3_873_s_247	11163273	A key feature of our model is that the binding of PDZ proteins to ct-GluR2/3 regulates the insertion of receptors.	bind
39575	1	10629	6	NULL	NULL	0	NULL	PDZ proteins	NULL		bind	NULL				ct-GluR2/3	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_28_3_873_s_247	11163273	A key feature of our model is that the binding of PDZ proteins to ct-GluR2/3 regulates the insertion of receptors.	bind
39576	2	10629	6	NULL	NULL	0	NULL	statement 1	NULL		regulates	NULL				receptors	NULL	insertion of 			NULL		0	NULL	NULL	NULL	gw60_neuron_28_3_873_s_247	11163273	A key feature of our model is that the binding of PDZ proteins to ct-GluR2/3 regulates the insertion of receptors.	bind
47254	1	10630	5	13	NULL	NULL	NULL	Atr	GP		bind					stalled replication forks	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_45507_s_163	14525986	A key feature of our studies is the observation that Cut5 is essential for the binding of both Atr and Pol alpha to stalled replication forks, two fundamental events in checkpoint activation.	bind
47255	2	10630	5	13	NULL	NULL	NULL	Cut5	GP		is essential for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_45507_s_163	14525986	A key feature of our studies is the observation that Cut5 is essential for the binding of both Atr and Pol alpha to stalled replication forks, two fundamental events in checkpoint activation.	bind
47256	3	10630	5	13	NULL	NULL	NULL	statement 1	Process		is a fundamental step in					checkpoint activation 	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_45507_s_163	14525986	A key feature of our studies is the observation that Cut5 is essential for the binding of both Atr and Pol alpha to stalled replication forks, two fundamental events in checkpoint activation.	bind
47257	4	10630	5	13	NULL	NULL	NULL	Pol alpha	GP		bind					stalled replication forks	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_45507_s_163	14525986	A key feature of our studies is the observation that Cut5 is essential for the binding of both Atr and Pol alpha to stalled replication forks, two fundamental events in checkpoint activation.	bind
47258	5	10630	5	13	NULL	NULL	NULL	Cut5	GP		is essential for					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_45507_s_163	14525986	A key feature of our studies is the observation that Cut5 is essential for the binding of both Atr and Pol alpha to stalled replication forks, two fundamental events in checkpoint activation.	bind
47259	6	10630	5	13	NULL	NULL	NULL	statement 4	Process		is a fundamental step in					checkpoint activation	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_45507_s_163	14525986	A key feature of our studies is the observation that Cut5 is essential for the binding of both Atr and Pol alpha to stalled replication forks, two fundamental events in checkpoint activation.	bind
39577	1	10630	6	NULL	NULL	0	NULL	Atr	NULL		bind	NULL				replication fork	NULL	stalled			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_45507_s_163	14525986	A key feature of our studies is the observation that Cut5 is essential for the binding of both Atr and Pol alpha to stalled replication forks, two fundamental events in checkpoint activation.	bind
39578	2	10630	6	NULL	NULL	0	NULL	Pol alpha	NULL		bind	NULL				replication fork	NULL	stalled			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_45507_s_163	14525986	A key feature of our studies is the observation that Cut5 is essential for the binding of both Atr and Pol alpha to stalled replication forks, two fundamental events in checkpoint activation.	bind
39579	3	10630	6	10	NULL	0	NULL	statement 1			is a fundamental step in					checkpoint activation					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_45507_s_163	14525986	A key feature of our studies is the observation that Cut5 is essential for the binding of both Atr and Pol alpha to stalled replication forks, two fundamental events in checkpoint activation.	bind
39580	4	10630	6	10	NULL	0	NULL	statement 2			is a fundamental step in					checkpoint activation					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_45507_s_163	14525986	A key feature of our studies is the observation that Cut5 is essential for the binding of both Atr and Pol alpha to stalled replication forks, two fundamental events in checkpoint activation.	bind
39581	5	10630	6	NULL	NULL	0	NULL	Cut5	NULL		is essential for	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_45507_s_163	14525986	A key feature of our studies is the observation that Cut5 is essential for the binding of both Atr and Pol alpha to stalled replication forks, two fundamental events in checkpoint activation.	bind
39582	6	10630	6	NULL	NULL	0	NULL	Cut5	NULL		is essential for	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_45507_s_163	14525986	A key feature of our studies is the observation that Cut5 is essential for the binding of both Atr and Pol alpha to stalled replication forks, two fundamental events in checkpoint activation.	bind
47260	1	10631	5	13	NULL	NULL	NULL	T cell	Cell		express					CD4	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_5_548_s_14	8805272	A key feature of the activation process is that the T cell can distinguish an MHC-bound ligand from other ligands because the T cell expresses cell-surface molecules, CD4 and CD8, which can bind directly to MHC proteins in domains distinct from their peptide-binding sites.	bind
47261	2	10631	5	13	NULL	NULL	NULL	CD4	GP		is a type of					cell-surface molecules	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_5_548_s_14	8805272	A key feature of the activation process is that the T cell can distinguish an MHC-bound ligand from other ligands because the T cell expresses cell-surface molecules, CD4 and CD8, which can bind directly to MHC proteins in domains distinct from their peptide-binding sites.	bind
47262	3	10631	5	13	NULL	NULL	NULL	CD4	GP		bind		directly			MHC proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_5_548_s_14	8805272	A key feature of the activation process is that the T cell can distinguish an MHC-bound ligand from other ligands because the T cell expresses cell-surface molecules, CD4 and CD8, which can bind directly to MHC proteins in domains distinct from their peptide-binding sites.	bind
47263	4	10631	5	13	NULL	NULL	NULL	T cells	Cell		express					CD8	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_5_548_s_14	8805272	A key feature of the activation process is that the T cell can distinguish an MHC-bound ligand from other ligands because the T cell expresses cell-surface molecules, CD4 and CD8, which can bind directly to MHC proteins in domains distinct from their peptide-binding sites.	bind
47264	5	10631	5	13	NULL	NULL	NULL	CD8	GP		is a type of					cell-surface molecules	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_5_548_s_14	8805272	A key feature of the activation process is that the T cell can distinguish an MHC-bound ligand from other ligands because the T cell expresses cell-surface molecules, CD4 and CD8, which can bind directly to MHC proteins in domains distinct from their peptide-binding sites.	bind
47265	6	10631	5	13	NULL	NULL	NULL	CD8	GP		bind		directly			MHC proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_6_5_548_s_14	8805272	A key feature of the activation process is that the T cell can distinguish an MHC-bound ligand from other ligands because the T cell expresses cell-surface molecules, CD4 and CD8, which can bind directly to MHC proteins in domains distinct from their peptide-binding sites.	bind
39583	1	10631	6	NULL	NULL	0	NULL	T cell	NULL		express	NULL				CD4	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_6_5_548_s_14	8805272	A key feature of the activation process is that the T cell can distinguish an MHC-bound ligand from other ligands because the T cell expresses cell-surface molecules, CD4 and CD8, which can bind directly to MHC proteins in domains distinct from their peptide-binding sites.	bind
39584	2	10631	6	NULL	NULL	0	NULL	T cell	NULL		express	NULL				CD8	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_6_5_548_s_14	8805272	A key feature of the activation process is that the T cell can distinguish an MHC-bound ligand from other ligands because the T cell expresses cell-surface molecules, CD4 and CD8, which can bind directly to MHC proteins in domains distinct from their peptide-binding sites.	bind
39585	3	10631	6	NULL	NULL	0	NULL	CD4 	NULL		is a type of	NULL				cell-surface molecule	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_6_5_548_s_14	8805272	A key feature of the activation process is that the T cell can distinguish an MHC-bound ligand from other ligands because the T cell expresses cell-surface molecules, CD4 and CD8, which can bind directly to MHC proteins in domains distinct from their peptide-binding sites.	bind
39586	4	10631	6	NULL	NULL	0	NULL	CD8	NULL		is a type of	NULL				cell surface receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_6_5_548_s_14	8805272	A key feature of the activation process is that the T cell can distinguish an MHC-bound ligand from other ligands because the T cell expresses cell-surface molecules, CD4 and CD8, which can bind directly to MHC proteins in domains distinct from their peptide-binding sites.	bind
39587	5	10631	6	NULL	NULL	0	NULL	CD4	NULL		bind	NULL	directly			MHC proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_6_5_548_s_14	8805272	A key feature of the activation process is that the T cell can distinguish an MHC-bound ligand from other ligands because the T cell expresses cell-surface molecules, CD4 and CD8, which can bind directly to MHC proteins in domains distinct from their peptide-binding sites.	bind
39588	6	10631	6	NULL	NULL	0	NULL	CD8	NULL		bind	NULL	directly			MHC proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_6_5_548_s_14	8805272	A key feature of the activation process is that the T cell can distinguish an MHC-bound ligand from other ligands because the T cell expresses cell-surface molecules, CD4 and CD8, which can bind directly to MHC proteins in domains distinct from their peptide-binding sites.	bind
47266	1	10632	5	13	NULL	NULL	NULL	EHD2	GP	acidic;;putative	 linked to		might be	Arp2/3 complex binding motif		actin cytoskeleton	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_11_10593_s_411	14676205	A key finding presented here is that at least two distinct motifs are present in the C terminus of EHD2 that might link this protein to the actin cytoskeleton, an acidic and putative Arp2/3 complex binding motif and the EH domain itself which binds the novel CH domain-containing protein EHBP1 (Figs.  6 and  10).	bind
47267	2	10632	5	13	NULL	NULL	NULL	EHD2	GP		 linked to		might be	EH domain		actin cytoskeleton	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_11_10593_s_411	14676205	A key finding presented here is that at least two distinct motifs are present in the C terminus of EHD2 that might link this protein to the actin cytoskeleton, an acidic and putative Arp2/3 complex binding motif and the EH domain itself which binds the novel CH domain-containing protein EHBP1 (Figs.  6 and  10).	bind
47268	3	10632	5	13	NULL	NULL	NULL				bind			EH domain		EHBP1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_11_10593_s_411	14676205	A key finding presented here is that at least two distinct motifs are present in the C terminus of EHD2 that might link this protein to the actin cytoskeleton, an acidic and putative Arp2/3 complex binding motif and the EH domain itself which binds the novel CH domain-containing protein EHBP1 (Figs.  6 and  10).	bind
47269	4	10632	5	13	NULL	NULL	NULL	EHBP1	GP		is a type of					CH domain-containing protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_11_10593_s_411	14676205	A key finding presented here is that at least two distinct motifs are present in the C terminus of EHD2 that might link this protein to the actin cytoskeleton, an acidic and putative Arp2/3 complex binding motif and the EH domain itself which binds the novel CH domain-containing protein EHBP1 (Figs.  6 and  10).	bind
39880	1	10632	6	NULL	NULL	0	NULL	EHD2 protein	NULL	acidic;; putative	linked to	NULL	might be	Arp2/3 complex binding motif in C-terminus		actin cytoskeleton	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_11_10593_s_411	14676205	A key finding presented here is that at least two distinct motifs are present in the C terminus of EHD2 that might link this protein to the actin cytoskeleton, an acidic and putative Arp2/3 complex binding motif and the EH domain itself which binds the novel CH domain-containing protein EHBP1 (Figs.  6 and  10).	bind
39881	2	10632	6	NULL	NULL	0	NULL	EHD2	NULL		linked to	NULL	might be	EH domain in C terminus		actin cytoskeleton	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_11_10593_s_411	14676205	A key finding presented here is that at least two distinct motifs are present in the C terminus of EHD2 that might link this protein to the actin cytoskeleton, an acidic and putative Arp2/3 complex binding motif and the EH domain itself which binds the novel CH domain-containing protein EHBP1 (Figs.  6 and  10).	bind
39882	3	10632	6	NULL	NULL	0	NULL	EHBP1	NULL		is a type of	NULL				CH domain-containing protein	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_11_10593_s_411	14676205	A key finding presented here is that at least two distinct motifs are present in the C terminus of EHD2 that might link this protein to the actin cytoskeleton, an acidic and putative Arp2/3 complex binding motif and the EH domain itself which binds the novel CH domain-containing protein EHBP1 (Figs.  6 and  10).	bind
39883	4	10632	6	NULL	NULL	0	NULL		NULL		bind	NULL		EH domain		EHBP1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_11_10593_s_411	14676205	A key finding presented here is that at least two distinct motifs are present in the C terminus of EHD2 that might link this protein to the actin cytoskeleton, an acidic and putative Arp2/3 complex binding motif and the EH domain itself which binds the novel CH domain-containing protein EHBP1 (Figs.  6 and  10).	bind
47270	1	10633	5	13	NULL	NULL	NULL	Ca2+	Chemical		mediates					feedback regulation	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_6_1097_s_16	11754840	A key mediator of the Ca2+-mediated feedback regulation is calmodulin   (Porter et al., 1995  ; Scott et al., 1997  ); however, there are only a few signaling proteins known to function in  Drosophila phototransduction that bind to calmodulin.	bind
50003	2	10633	5	13	NULL	NULL	NULL	calmodulin	GP		key mediator of					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_6_1097_s_16	11754840	A key mediator of the Ca2+-mediated feedback regulation is calmodulin   (Porter et al., 1995  ; Scott et al., 1997  ); however, there are only a few signaling proteins known to function in  Drosophila phototransduction that bind to calmodulin.	bind
50005	3	10633	5	13	NULL	NULL	NULL	signaling proteins	GP		function in					 phototransduction 	Process	Drosophila			NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_6_1097_s_16	11754840	A key mediator of the Ca2+-mediated feedback regulation is calmodulin   (Porter et al., 1995  ; Scott et al., 1997  ); however, there are only a few signaling proteins known to function in  Drosophila phototransduction that bind to calmodulin.	bind
50006	4	10633	5	13	NULL	NULL	NULL	statement 3	GP		bind					calmodulin	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_6_1097_s_16	11754840	A key mediator of the Ca2+-mediated feedback regulation is calmodulin   (Porter et al., 1995  ; Scott et al., 1997  ); however, there are only a few signaling proteins known to function in  Drosophila phototransduction that bind to calmodulin.	bind
39589	1	10633	6	10	NULL	0	NULL	Ca2+	NULL		mediates	NULL				feedback regulation	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_6_1097_s_16	11754840	A key mediator of the Ca2+-mediated feedback regulation is calmodulin   (Porter et al., 1995  ; Scott et al., 1997  ); however, there are only a few signaling proteins known to function in  Drosophila phototransduction that bind to calmodulin.	bind
50004	2	10633	6	10	NULL	0	NULL	calmodulin	NULL		key mediator of	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuron_32_6_1097_s_16	11754840	A key mediator of the Ca2+-mediated feedback regulation is calmodulin   (Porter et al., 1995  ; Scott et al., 1997  ); however, there are only a few signaling proteins known to function in  Drosophila phototransduction that bind to calmodulin.	bind
50007	3	10633	6	10	NULL	0	NULL	signaling proteins	NULL		function in	NULL				phototransduction	NULL	Drosophila			NULL		0	NULL	NULL	NULL	gw60_neuron_32_6_1097_s_16	11754840	A key mediator of the Ca2+-mediated feedback regulation is calmodulin   (Porter et al., 1995  ; Scott et al., 1997  ); however, there are only a few signaling proteins known to function in  Drosophila phototransduction that bind to calmodulin.	bind
50008	4	10633	6	10	NULL	0	NULL	statement 3	NULL		bind	NULL				calmodulin	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_32_6_1097_s_16	11754840	A key mediator of the Ca2+-mediated feedback regulation is calmodulin   (Porter et al., 1995  ; Scott et al., 1997  ); however, there are only a few signaling proteins known to function in  Drosophila phototransduction that bind to calmodulin.	bind
47271	1	10634	5	13	NULL	NULL	NULL	TGFalpha	GP		is a type of					mitogenic peptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_52_33181_s_243	9407106	A key mitogenic peptide involved in squamous epithelial proliferation is TGFalpha, which is believed to be more physiologically relevant in these tissues than epidermal growth factor, although both bind the same epidermal growth factor receptor ( 30,  44).	bind
47272	2	10634	5	13	NULL	NULL	NULL	TGFalpha	GP		is involved in					squamous epithelium	OrganismPart	proliferation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_52_33181_s_243	9407106	A key mitogenic peptide involved in squamous epithelial proliferation is TGFalpha, which is believed to be more physiologically relevant in these tissues than epidermal growth factor, although both bind the same epidermal growth factor receptor ( 30,  44).	bind
47275	3	10634	5	13	NULL	NULL	NULL	TGFalpha	GP		bind					epidermal growth factor receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_52_33181_s_243	9407106	A key mitogenic peptide involved in squamous epithelial proliferation is TGFalpha, which is believed to be more physiologically relevant in these tissues than epidermal growth factor, although both bind the same epidermal growth factor receptor ( 30,  44).	bind
47277	4	10634	5	13	NULL	NULL	NULL	epidermal growth factor	GP		bind					epidermal growth factor receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_52_33181_s_243	9407106	A key mitogenic peptide involved in squamous epithelial proliferation is TGFalpha, which is believed to be more physiologically relevant in these tissues than epidermal growth factor, although both bind the same epidermal growth factor receptor ( 30,  44).	bind
39590	1	10634	6	10	NULL	0	NULL	TGFalpha			plays a role in					squamous epithelial		proliferation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_52_33181_s_243	9407106	A key mitogenic peptide involved in squamous epithelial proliferation is TGFalpha, which is believed to be more physiologically relevant in these tissues than epidermal growth factor, although both bind the same epidermal growth factor receptor ( 30,  44).	bind
39884	2	10634	6	NULL	NULL	0	NULL	TGFalpha	NULL		bind	NULL				epidermal growth factor receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_52_33181_s_243	9407106	A key mitogenic peptide involved in squamous epithelial proliferation is TGFalpha, which is believed to be more physiologically relevant in these tissues than epidermal growth factor, although both bind the same epidermal growth factor receptor ( 30,  44).	bind
39885	3	10634	6	NULL	NULL	0	NULL	epidermal growth factor	NULL		bind	NULL				epidermal growth factor receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_52_33181_s_243	9407106	A key mitogenic peptide involved in squamous epithelial proliferation is TGFalpha, which is believed to be more physiologically relevant in these tissues than epidermal growth factor, although both bind the same epidermal growth factor receptor ( 30,  44).	bind
50009	4	10634	6	10	NULL	0	NULL	TGFalpha	NULL		is a type of	NULL				mitogenic peptide	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_52_33181_s_243	9407106	A key mitogenic peptide involved in squamous epithelial proliferation is TGFalpha, which is believed to be more physiologically relevant in these tissues than epidermal growth factor, although both bind the same epidermal growth factor receptor ( 30,  44).	bind
47282	1	10635	5	13	NULL	NULL	NULL	hHop	GP		forms chimera with							Drosophila	DP2		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_10_8906_s_187	15632128	A key observation in this study is that exchanging DP2 between hHop and dHop does not grossly affect Hsp70 binding; nonetheless, chimera I (hHop with  Drosophila DP2) fails to support GR activity, and the converse chimera J (dHop with human DP2) gains the ability to enhance GR activity.	bind
47283	2	10635	5	13	NULL	NULL	NULL	statement 1	Process		does not support					GR	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_10_8906_s_187	15632128	A key observation in this study is that exchanging DP2 between hHop and dHop does not grossly affect Hsp70 binding; nonetheless, chimera I (hHop with  Drosophila DP2) fails to support GR activity, and the converse chimera J (dHop with human DP2) gains the ability to enhance GR activity.	bind
47284	3	10635	5	13	NULL	NULL	NULL	dHop	GP		forms chimera with							human	DP2		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_10_8906_s_187	15632128	A key observation in this study is that exchanging DP2 between hHop and dHop does not grossly affect Hsp70 binding; nonetheless, chimera I (hHop with  Drosophila DP2) fails to support GR activity, and the converse chimera J (dHop with human DP2) gains the ability to enhance GR activity.	bind
47285	4	10635	5	13	NULL	NULL	NULL	statement 3	Process		enhance					GR	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_10_8906_s_187	15632128	A key observation in this study is that exchanging DP2 between hHop and dHop does not grossly affect Hsp70 binding; nonetheless, chimera I (hHop with  Drosophila DP2) fails to support GR activity, and the converse chimera J (dHop with human DP2) gains the ability to enhance GR activity.	bind
39983	1	10635	6	NULL	NULL	0	NULL	Hop	NULL	human	forms a chimeric protein with	NULL					NULL	Drosophila	DP2		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8906_s_187	15632128	A key observation in this study is that exchanging DP2 between hHop and dHop does not grossly affect Hsp70 binding; nonetheless, chimera I (hHop with  Drosophila DP2) fails to support GR activity, and the converse chimera J (dHop with human DP2) gains the ability to enhance GR activity.	bind
39984	2	10635	6	NULL	NULL	0	NULL	statement 1	NULL		does not support	NULL				GR	NULL	activity of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8906_s_187	15632128	A key observation in this study is that exchanging DP2 between hHop and dHop does not grossly affect Hsp70 binding; nonetheless, chimera I (hHop with  Drosophila DP2) fails to support GR activity, and the converse chimera J (dHop with human DP2) gains the ability to enhance GR activity.	bind
39985	3	10635	6	NULL	NULL	0	NULL	Hop	NULL	Drosophila	forms a chimeric protein with	NULL					NULL	human	DP2		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8906_s_187	15632128	A key observation in this study is that exchanging DP2 between hHop and dHop does not grossly affect Hsp70 binding; nonetheless, chimera I (hHop with  Drosophila DP2) fails to support GR activity, and the converse chimera J (dHop with human DP2) gains the ability to enhance GR activity.	bind
39986	4	10635	6	NULL	NULL	0	NULL	statement 3	NULL		enhances	NULL				GR	NULL	activity of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8906_s_187	15632128	A key observation in this study is that exchanging DP2 between hHop and dHop does not grossly affect Hsp70 binding; nonetheless, chimera I (hHop with  Drosophila DP2) fails to support GR activity, and the converse chimera J (dHop with human DP2) gains the ability to enhance GR activity.	bind
47286	1	10636	5	13	NULL	NULL	NULL	Rb protein	GP		is					retinoblastoma protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_15_6560_s_17	15254224	A key physiological substrate for Cdk4 and Cdk6 is the retinoblastoma (Rb) protein, which binds and inactivates the E2F-DP transcription complexes that are essential for S-phase entry.	bind
47287	2	10636	5	13	NULL	NULL	NULL	Rb protein	GP		is a physiological substrate for					Cdk4	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_15_6560_s_17	15254224	A key physiological substrate for Cdk4 and Cdk6 is the retinoblastoma (Rb) protein, which binds and inactivates the E2F-DP transcription complexes that are essential for S-phase entry.	bind
47288	3	10636	5	13	NULL	NULL	NULL	Rb protein	GP		is a physiological substrate for					Cdk6	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_15_6560_s_17	15254224	A key physiological substrate for Cdk4 and Cdk6 is the retinoblastoma (Rb) protein, which binds and inactivates the E2F-DP transcription complexes that are essential for S-phase entry.	bind
47290	4	10636	5	13	NULL	NULL	NULL	Rb protein	GP		bind					E2F-DP transcription complexes	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_15_6560_s_17	15254224	A key physiological substrate for Cdk4 and Cdk6 is the retinoblastoma (Rb) protein, which binds and inactivates the E2F-DP transcription complexes that are essential for S-phase entry.	bind
47291	5	10636	5	13	NULL	NULL	NULL	statement 4	Process		inactivates					E2F-DP transcription complexes	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_15_6560_s_17	15254224	A key physiological substrate for Cdk4 and Cdk6 is the retinoblastoma (Rb) protein, which binds and inactivates the E2F-DP transcription complexes that are essential for S-phase entry.	bind
47293	6	10636	5	13	NULL	NULL	NULL	E2F-DP transcription complexes	GP		is essential for					S-phase	Process	entry into			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_15_6560_s_17	15254224	A key physiological substrate for Cdk4 and Cdk6 is the retinoblastoma (Rb) protein, which binds and inactivates the E2F-DP transcription complexes that are essential for S-phase entry.	bind
39591	1	10636	6	NULL	NULL	0	NULL	Rb protein	NULL		is the physiological substrate for	NULL				Cdk4	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_15_6560_s_17	15254224	A key physiological substrate for Cdk4 and Cdk6 is the retinoblastoma (Rb) protein, which binds and inactivates the E2F-DP transcription complexes that are essential for S-phase entry.	bind
39592	2	10636	6	NULL	NULL	0	NULL	Rb protein	NULL		is the physiological substrate for	NULL				Cdk6	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_15_6560_s_17	15254224	A key physiological substrate for Cdk4 and Cdk6 is the retinoblastoma (Rb) protein, which binds and inactivates the E2F-DP transcription complexes that are essential for S-phase entry.	bind
39593	3	10636	6	NULL	NULL	0	NULL	Rb	NULL		is	NULL				retinoblastoma protein	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_15_6560_s_17	15254224	A key physiological substrate for Cdk4 and Cdk6 is the retinoblastoma (Rb) protein, which binds and inactivates the E2F-DP transcription complexes that are essential for S-phase entry.	bind
39594	4	10636	6	NULL	NULL	0	NULL	E2F-DP transcription complexes	NULL		are essential for	NULL				S-phase	NULL	entry into			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_15_6560_s_17	15254224	A key physiological substrate for Cdk4 and Cdk6 is the retinoblastoma (Rb) protein, which binds and inactivates the E2F-DP transcription complexes that are essential for S-phase entry.	bind
39595	5	10636	6	NULL	NULL	0	NULL	Rb protein	NULL		bind	NULL				E2F-DP transcription complexes	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_15_6560_s_17	15254224	A key physiological substrate for Cdk4 and Cdk6 is the retinoblastoma (Rb) protein, which binds and inactivates the E2F-DP transcription complexes that are essential for S-phase entry.	bind
39596	6	10636	6	NULL	NULL	0	NULL	Rb protein	NULL		inactivates	NULL				E2F-DP transcription complexes	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_15_6560_s_17	15254224	A key physiological substrate for Cdk4 and Cdk6 is the retinoblastoma (Rb) protein, which binds and inactivates the E2F-DP transcription complexes that are essential for S-phase entry.	bind
47294	1	10637	5	13	NULL	NULL	NULL	CcmE	GP		is a type of					heme chaperone	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_35_32591_s_24	11384983	A key player in the maturation pathway has been identified in the heme chaperone CcmE, which binds heme covalently at a single histidine residue and subsequently transfers it to apocytochrome  c ( 11).	bind
47295	2	10637	5	13	NULL	NULL	NULL	CcmE	GP		bind		covalently			heme	Chemical		histidine residue		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_35_32591_s_24	11384983	A key player in the maturation pathway has been identified in the heme chaperone CcmE, which binds heme covalently at a single histidine residue and subsequently transfers it to apocytochrome  c ( 11).	bind
47296	3	10637	5	13	NULL	NULL	NULL	heme	Chemical		is transfered to					apocytochrome c	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_35_32591_s_24	11384983	A key player in the maturation pathway has been identified in the heme chaperone CcmE, which binds heme covalently at a single histidine residue and subsequently transfers it to apocytochrome  c ( 11).	bind
47297	4	10637	5	13	NULL	NULL	NULL	statement 2	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_35_32591_s_24	11384983	A key player in the maturation pathway has been identified in the heme chaperone CcmE, which binds heme covalently at a single histidine residue and subsequently transfers it to apocytochrome  c ( 11).	bind
39597	1	10637	6	NULL	NULL	0	NULL	CcmE	NULL		is a type of	NULL				heme chaperone	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_35_32591_s_24	11384983	A key player in the maturation pathway has been identified in the heme chaperone CcmE, which binds heme covalently at a single histidine residue and subsequently transfers it to apocytochrome  c ( 11).	bind
39598	2	10637	6	NULL	NULL	0	NULL	CcmE	NULL		bind	NULL	covalently			heme	NULL		histidine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_35_32591_s_24	11384983	A key player in the maturation pathway has been identified in the heme chaperone CcmE, which binds heme covalently at a single histidine residue and subsequently transfers it to apocytochrome  c ( 11).	bind
39599	3	10637	6	NULL	NULL	0	NULL	heme	NULL		is transfered to	NULL				apocytochrome c	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_35_32591_s_24	11384983	A key player in the maturation pathway has been identified in the heme chaperone CcmE, which binds heme covalently at a single histidine residue and subsequently transfers it to apocytochrome  c ( 11).	bind
39600	4	10637	6	NULL	NULL	0	NULL	CcmE	NULL		transfers	NULL				heme	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_35_32591_s_24	11384983	A key player in the maturation pathway has been identified in the heme chaperone CcmE, which binds heme covalently at a single histidine residue and subsequently transfers it to apocytochrome  c ( 11).	bind
39601	5	10637	6	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_35_32591_s_24	11384983	A key player in the maturation pathway has been identified in the heme chaperone CcmE, which binds heme covalently at a single histidine residue and subsequently transfers it to apocytochrome  c ( 11).	bind
47298	1	10638	5	13	NULL	NULL	NULL	v-Src	GP		mediates					STAT3	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2043_s_50	10688651	A key question, then, is how v-Src or activated c-Src mediates the activation of STAT3.	bind
47299	2	10638	5	13	NULL	NULL	NULL	c-Src	GP	activated	mediates					STAT3	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_2043_s_50	10688651	A key question, then, is how v-Src or activated c-Src mediates the activation of STAT3.	bind
39602	1	10638	6	NULL	NULL	0	NULL	v-Src	NULL		mediates	NULL				STAT3	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_6_2043_s_50	10688651	A key question, then, is how v-Src or activated c-Src mediates the activation of STAT3.	bind
39603	2	10638	6	NULL	NULL	0	NULL	c-Src	NULL	activated	mediates	NULL				STAT3	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_6_2043_s_50	10688651	A key question, then, is how v-Src or activated c-Src mediates the activation of STAT3.	bind
47300	1	10639	5	13	NULL	NULL	NULL	Fas	GP		bind					FasL	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_49_40599_s_18	16227629	A key signaling activity of Fas, which binds to Fas ligand (FasL), and of DR4 and DR5, which bind to Apo2L/TRAIL, is apoptosis induction.	bind
47301	2	10639	5	13	NULL	NULL	NULL	FasL	GP		is					Fas ligand	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_49_40599_s_18	16227629	A key signaling activity of Fas, which binds to Fas ligand (FasL), and of DR4 and DR5, which bind to Apo2L/TRAIL, is apoptosis induction.	bind
47302	3	10639	5	13	NULL	NULL	NULL	DR4	GP		bind					Apo2L/TRAIL	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_49_40599_s_18	16227629	A key signaling activity of Fas, which binds to Fas ligand (FasL), and of DR4 and DR5, which bind to Apo2L/TRAIL, is apoptosis induction.	bind
47303	4	10639	5	13	NULL	NULL	NULL	DR5	GP		bind					Apo2L/TRAIL	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_49_40599_s_18	16227629	A key signaling activity of Fas, which binds to Fas ligand (FasL), and of DR4 and DR5, which bind to Apo2L/TRAIL, is apoptosis induction.	bind
47304	5	10639	5	13	NULL	NULL	NULL	apoptosis	Process	induction of	is a key signaling activity of					Fas	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_49_40599_s_18	16227629	A key signaling activity of Fas, which binds to Fas ligand (FasL), and of DR4 and DR5, which bind to Apo2L/TRAIL, is apoptosis induction.	bind
47305	6	10639	5	13	NULL	NULL	NULL	apoptosis	Process	induction of	is a key signaling activity of					DR4	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_49_40599_s_18	16227629	A key signaling activity of Fas, which binds to Fas ligand (FasL), and of DR4 and DR5, which bind to Apo2L/TRAIL, is apoptosis induction.	bind
47307	7	10639	5	13	NULL	NULL	NULL	apoptosis	Process	induction of	is a key signaling activity of					DR5	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_49_40599_s_18	16227629	A key signaling activity of Fas, which binds to Fas ligand (FasL), and of DR4 and DR5, which bind to Apo2L/TRAIL, is apoptosis induction.	bind
39604	1	10639	6	NULL	NULL	0	NULL	Fas	NULL		bind	NULL				FasL	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_49_40599_s_18	16227629	A key signaling activity of Fas, which binds to Fas ligand (FasL), and of DR4 and DR5, which bind to Apo2L/TRAIL, is apoptosis induction.	bind
39605	2	10639	6	NULL	NULL	0	NULL	DR4	NULL		bind	NULL				Apo2L/TRAIL	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_49_40599_s_18	16227629	A key signaling activity of Fas, which binds to Fas ligand (FasL), and of DR4 and DR5, which bind to Apo2L/TRAIL, is apoptosis induction.	bind
39606	3	10639	6	NULL	NULL	0	NULL	DR5	NULL		bind	NULL				Apo2L/TRAIL	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_49_40599_s_18	16227629	A key signaling activity of Fas, which binds to Fas ligand (FasL), and of DR4 and DR5, which bind to Apo2L/TRAIL, is apoptosis induction.	bind
39607	4	10639	6	NULL	NULL	0	NULL	Fas	NULL		plays a role in	NULL				apoptosis	NULL	induction of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_49_40599_s_18	16227629	A key signaling activity of Fas, which binds to Fas ligand (FasL), and of DR4 and DR5, which bind to Apo2L/TRAIL, is apoptosis induction.	bind
39608	5	10639	6	NULL	NULL	0	NULL	DR4	NULL		plays a role in	NULL				apoptosis	NULL	induction of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_49_40599_s_18	16227629	A key signaling activity of Fas, which binds to Fas ligand (FasL), and of DR4 and DR5, which bind to Apo2L/TRAIL, is apoptosis induction.	bind
39609	6	10639	6	NULL	NULL	0	NULL	DR5	NULL		plays a role in	NULL				apoptosis	NULL	induction of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_49_40599_s_18	16227629	A key signaling activity of Fas, which binds to Fas ligand (FasL), and of DR4 and DR5, which bind to Apo2L/TRAIL, is apoptosis induction.	bind
50010	7	10639	6	10	NULL	0	NULL	FasL	NULL		is	NULL				Fas ligand	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_49_40599_s_18	16227629	A key signaling activity of Fas, which binds to Fas ligand (FasL), and of DR4 and DR5, which bind to Apo2L/TRAIL, is apoptosis induction.	bind
47309	1	10640	5	13	NULL	NULL	NULL	MHC I	GP		bind					CD8	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_15_0_535_s_196	9143699	A key to understanding coreceptor expression by NK1 T cells is whether CD1 binds CD8  (as does MHC I), or CD4 (like MHC II), or neither.	bind
47310	2	10640	5	13	NULL	NULL	NULL	MHC II	GP		bind					CD4	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_15_0_535_s_196	9143699	A key to understanding coreceptor expression by NK1 T cells is whether CD1 binds CD8  (as does MHC I), or CD4 (like MHC II), or neither.	bind
39610	1	10640	6	NULL	NULL	0	NULL	MHC I	NULL		bind	NULL				CD8	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_15_0_535_s_196	9143699	A key to understanding coreceptor expression by NK1 T cells is whether CD1 binds CD8  (as does MHC I), or CD4 (like MHC II), or neither.	bind
39611	2	10640	6	NULL	NULL	0	NULL	MHC II	NULL		bind	NULL				CD4	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_15_0_535_s_196	9143699	A key to understanding coreceptor expression by NK1 T cells is whether CD1 binds CD8  (as does MHC I), or CD4 (like MHC II), or neither.	bind
47313	1	10641	5	13	NULL	NULL	NULL	p27	GP	mutant	bind			kinase		cyclins	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_21_20620_s_214	15788393	A kinase contact mutant of p27, which still binds cyclins, does not inhibit cyclin E-cdk2 complexes but becomes phosphorylated and rapidly degraded.	bind
47314	2	10641	5	13	NULL	NULL	NULL	p27	GP	mutant	does not inhibit			kinase		cyclin E-cdk2 complexes	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_21_20620_s_214	15788393	A kinase contact mutant of p27, which still binds cyclins, does not inhibit cyclin E-cdk2 complexes but becomes phosphorylated and rapidly degraded.	bind
47316	3	10641	5	13	NULL	NULL	NULL	p27	GP	mutant	undergoes			kinase		phosphorylation	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_21_20620_s_214	15788393	A kinase contact mutant of p27, which still binds cyclins, does not inhibit cyclin E-cdk2 complexes but becomes phosphorylated and rapidly degraded.	bind
47318	4	10641	5	13	NULL	NULL	NULL	p27	GP	mutant	undergoes		rapidly	kinase		degradation	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_21_20620_s_214	15788393	A kinase contact mutant of p27, which still binds cyclins, does not inhibit cyclin E-cdk2 complexes but becomes phosphorylated and rapidly degraded.	bind
39612	1	10641	6	NULL	NULL	0	NULL	p27	NULL	mutant	bind	NULL		kinase		cyclin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_21_20620_s_214	15788393	A kinase contact mutant of p27, which still binds cyclins, does not inhibit cyclin E-cdk2 complexes but becomes phosphorylated and rapidly degraded.	bind
39613	2	10641	6	NULL	NULL	0	NULL	p27	NULL	mutant	does not inhibit	NULL		kinase		cyclin E-cdk2 complexes	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_21_20620_s_214	15788393	A kinase contact mutant of p27, which still binds cyclins, does not inhibit cyclin E-cdk2 complexes but becomes phosphorylated and rapidly degraded.	bind
39614	3	10641	6	10	NULL	0	NULL	p27	NULL	mutant	undergoes	NULL	rapidly	kinase		degradation	NULL	rapidly			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_21_20620_s_214	15788393	A kinase contact mutant of p27, which still binds cyclins, does not inhibit cyclin E-cdk2 complexes but becomes phosphorylated and rapidly degraded.	bind
39615	4	10641	6	10	NULL	0	NULL	p27	NULL	mutant	undergoes	NULL		kinase		phosphorylation	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_21_20620_s_214	15788393	A kinase contact mutant of p27, which still binds cyclins, does not inhibit cyclin E-cdk2 complexes but becomes phosphorylated and rapidly degraded.	bind
47321	1	10642	5	13	NULL	NULL	NULL	kinase	GP	human;;platelets	bind					RalA	GP	recombinant			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1763_9_948_s_132	16945434	A kinase from human platelets binds to recombinant RalA and RalB. 200  l GST-RalA-GDP  or GST-RalB-GDP or GST-cH-Ras-GDP bead suspension (1:1) was incubated with total  human platelet extract.	bind
47322	2	10642	5	13	NULL	NULL	NULL	kinase	GP	human;;platelets	bind					RalB	GP	recombinant			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1763_9_948_s_132	16945434	A kinase from human platelets binds to recombinant RalA and RalB. 200  l GST-RalA-GDP  or GST-RalB-GDP or GST-cH-Ras-GDP bead suspension (1:1) was incubated with total  human platelet extract.	bind
39616	1	10642	6	NULL	NULL	0	NULL	kinase 	NULL	 human;; platelets	bind	NULL				RalA	NULL	recombinant			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1763_9_948_s_132	16945434	A kinase from human platelets binds to recombinant RalA and RalB. 200  l GST-RalA-GDP  or GST-RalB-GDP or GST-cH-Ras-GDP bead suspension (1:1) was incubated with total  human platelet extract.	bind
39617	2	10642	6	NULL	NULL	0	NULL	kinase	NULL	human;; platelets	bind	NULL				RalB	NULL	recombinant			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1763_9_948_s_132	16945434	A kinase from human platelets binds to recombinant RalA and RalB. 200  l GST-RalA-GDP  or GST-RalB-GDP or GST-cH-Ras-GDP bead suspension (1:1) was incubated with total  human platelet extract.	bind
47324	1	10643	5	13	NULL	NULL	NULL	PHAS-I	GP		bind					eIF-4E	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_31_18531_s_266	7629182	A kinase that acted on both free  [H ]PHAS-I and [H ]PHAS-I  bound to eIF-4E eluted at relatively high concentrations of NaCl  (fraction 58).	bind
39618	1	10643	6	NULL	NULL	0	NULL	PHAS-I 	NULL		bind	NULL				eIF-4E	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_31_18531_s_266	7629182	A kinase that acted on both free  [H ]PHAS-I and [H ]PHAS-I  bound to eIF-4E eluted at relatively high concentrations of NaCl  (fraction 58).	bind
47325	1	10644	5	13	NULL	NULL	NULL	PDK1	GP		is a type of					kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_31_22033_s_140	10419529	A kinase, termed PDK1, that can phosphorylate Thr-308 only when Akt/PKB is bound to PIP3 has been purified and cloned.	bind
47327	2	10644	5	13	NULL	NULL	NULL	Akt/PKB	GP		bind					PIP3	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_31_22033_s_140	10419529	A kinase, termed PDK1, that can phosphorylate Thr-308 only when Akt/PKB is bound to PIP3 has been purified and cloned.	bind
47328	3	10644	5	13	NULL	NULL	NULL	PDK1	GP		phosphorylate								Thr-308		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_31_22033_s_140	10419529	A kinase, termed PDK1, that can phosphorylate Thr-308 only when Akt/PKB is bound to PIP3 has been purified and cloned.	bind
47332	4	10644	5	13	NULL	NULL	NULL	statement 3	Process		in the presence of		only			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_31_22033_s_140	10419529	A kinase, termed PDK1, that can phosphorylate Thr-308 only when Akt/PKB is bound to PIP3 has been purified and cloned.	bind
39775	1	10644	6	NULL	NULL	0	NULL	Akt/PKB	NULL		bind	NULL				PIP3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_31_22033_s_140	10419529	A kinase, termed PDK1, that can phosphorylate Thr-308 only when Akt/PKB is bound to PIP3 has been purified and cloned.	bind
39776	2	10644	6	NULL	NULL	0	NULL	PDK1	NULL		is a type of	NULL				kinase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_31_22033_s_140	10419529	A kinase, termed PDK1, that can phosphorylate Thr-308 only when Akt/PKB is bound to PIP3 has been purified and cloned.	bind
39777	3	10644	6	NULL	NULL	0	NULL	PDK1	NULL		phosphorylates	NULL					NULL		Thr-308		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_31_22033_s_140	10419529	A kinase, termed PDK1, that can phosphorylate Thr-308 only when Akt/PKB is bound to PIP3 has been purified and cloned.	bind
39778	4	10644	6	10	NULL	0	NULL	statement 3	NULL		occurs upon	NULL	only			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_31_22033_s_140	10419529	A kinase, termed PDK1, that can phosphorylate Thr-308 only when Akt/PKB is bound to PIP3 has been purified and cloned.	bind
47333	1	10647	5	13	NULL	NULL	NULL	Kidins220	GP		is localized to					plasma membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_281_27_16651260_s_5	16651260	A kinase-inactive mutant of PKD3 is only able to alter the localization  of Kidins220 at the plasma membrane when its C terminus has been substituted  by the PDZ-binding motif of PKD1 or PKD2.	bind
47334	2	10647	5	13	NULL	NULL	NULL	PKD3	GP		is substituted by			C terminus		PKD1	GP		PDZ-binding motif		NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_281_27_16651260_s_5	16651260	A kinase-inactive mutant of PKD3 is only able to alter the localization  of Kidins220 at the plasma membrane when its C terminus has been substituted  by the PDZ-binding motif of PKD1 or PKD2.	bind
47336	3	10647	5	13	NULL	NULL	NULL	PKD3	GP		is substituted by			carboxyl terminus		PKD2	GP		PDZ-binding motif		NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_281_27_16651260_s_5	16651260	A kinase-inactive mutant of PKD3 is only able to alter the localization  of Kidins220 at the plasma membrane when its C terminus has been substituted  by the PDZ-binding motif of PKD1 or PKD2.	bind
47338	4	10647	5	13	NULL	NULL	NULL	statement 2	Process		alters					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_281_27_16651260_s_5	16651260	A kinase-inactive mutant of PKD3 is only able to alter the localization  of Kidins220 at the plasma membrane when its C terminus has been substituted  by the PDZ-binding motif of PKD1 or PKD2.	bind
47339	5	10647	5	13	NULL	NULL	NULL	statement 3	Process		alters					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_281_27_16651260_s_5	16651260	A kinase-inactive mutant of PKD3 is only able to alter the localization  of Kidins220 at the plasma membrane when its C terminus has been substituted  by the PDZ-binding motif of PKD1 or PKD2.	bind
39886	1	10647	6	NULL	NULL	0	NULL	Kidins220	NULL		is localized at	NULL				plasma membrane	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_281_27_16651260_s_5	16651260	A kinase-inactive mutant of PKD3 is only able to alter the localization  of Kidins220 at the plasma membrane when its C terminus has been substituted  by the PDZ-binding motif of PKD1 or PKD2.	bind
39887	2	10647	6	NULL	NULL	0	NULL	PKD3	NULL		is substituted by	NULL		C-terminus		PKD1	NULL		PDZ-binding motif		NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_281_27_16651260_s_5	16651260	A kinase-inactive mutant of PKD3 is only able to alter the localization  of Kidins220 at the plasma membrane when its C terminus has been substituted  by the PDZ-binding motif of PKD1 or PKD2.	bind
39888	3	10647	6	NULL	NULL	0	NULL	PKD3	NULL		is substituted by	NULL		C terminus		PKD2	NULL		PDZ-binding motif		NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_281_27_16651260_s_5	16651260	A kinase-inactive mutant of PKD3 is only able to alter the localization  of Kidins220 at the plasma membrane when its C terminus has been substituted  by the PDZ-binding motif of PKD1 or PKD2.	bind
39940	4	10647	6	NULL	NULL	0	NULL	statement 2	NULL		alters	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_281_27_16651260_s_5	16651260	A kinase-inactive mutant of PKD3 is only able to alter the localization  of Kidins220 at the plasma membrane when its C terminus has been substituted  by the PDZ-binding motif of PKD1 or PKD2.	bind
39941	5	10647	6	NULL	NULL	0	NULL	statement 3	NULL		alters	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_281_27_16651260_s_5	16651260	A kinase-inactive mutant of PKD3 is only able to alter the localization  of Kidins220 at the plasma membrane when its C terminus has been substituted  by the PDZ-binding motif of PKD1 or PKD2.	bind
47340	1	10648	5	13	NULL	NULL	NULL	kinectin isoform	GP		lacks							major portion of	kinesin-binding domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_34_32115_s_3	12773547	A kinectin isoform that lacks a major portion of the  kinesin-binding domain does not bind kinesin but interacts with another  resident of the endoplasmic reticulum, the translation elongation factor-1  delta (EF-1delta).	bind
47341	2	10648	5	13	NULL	NULL	NULL	statement 1	GP		does not bind					kinesin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_34_32115_s_3	12773547	A kinectin isoform that lacks a major portion of the  kinesin-binding domain does not bind kinesin but interacts with another  resident of the endoplasmic reticulum, the translation elongation factor-1  delta (EF-1delta).	bind
47342	3	10648	5	13	NULL	NULL	NULL	statement 1	GP		interacts with					EF-1delta	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_34_32115_s_3	12773547	A kinectin isoform that lacks a major portion of the  kinesin-binding domain does not bind kinesin but interacts with another  resident of the endoplasmic reticulum, the translation elongation factor-1  delta (EF-1delta).	bind
47343	4	10648	5	13	NULL	NULL	NULL	EF-1delta	GP		is					translation elongation factor-1 delta	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_34_32115_s_3	12773547	A kinectin isoform that lacks a major portion of the  kinesin-binding domain does not bind kinesin but interacts with another  resident of the endoplasmic reticulum, the translation elongation factor-1  delta (EF-1delta).	bind
47344	5	10648	5	13	NULL	NULL	NULL	EF-1delta	GP		resides in					endoplasmic reticulum	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_34_32115_s_3	12773547	A kinectin isoform that lacks a major portion of the  kinesin-binding domain does not bind kinesin but interacts with another  resident of the endoplasmic reticulum, the translation elongation factor-1  delta (EF-1delta).	bind
39779	5	10648	6	10	NULL	0	NULL	statement 1	NULL		does not bind	NULL				kinesin	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_34_32115_s_3	12773547	A kinectin isoform that lacks a major portion of the  kinesin-binding domain does not bind kinesin but interacts with another  resident of the endoplasmic reticulum, the translation elongation factor-1  delta (EF-1delta).	bind
39780	2	10648	6	10	NULL	0	NULL	statement 1	NULL		interacts with	NULL				translation EF-1delta	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_34_32115_s_3	12773547	A kinectin isoform that lacks a major portion of the  kinesin-binding domain does not bind kinesin but interacts with another  resident of the endoplasmic reticulum, the translation elongation factor-1  delta (EF-1delta).	bind
39781	3	10648	6	NULL	NULL	0	NULL	EF-1delta	NULL		is	NULL				elongation factor-1 delta	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_32115_s_3	12773547	A kinectin isoform that lacks a major portion of the  kinesin-binding domain does not bind kinesin but interacts with another  resident of the endoplasmic reticulum, the translation elongation factor-1  delta (EF-1delta).	bind
39782	4	10648	6	NULL	NULL	0	NULL	EF-1delta	NULL		resides in	NULL				endoplasmic reticulum	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_32115_s_3	12773547	A kinectin isoform that lacks a major portion of the  kinesin-binding domain does not bind kinesin but interacts with another  resident of the endoplasmic reticulum, the translation elongation factor-1  delta (EF-1delta).	bind
50011	1	10648	6	10	NULL	0	NULL	kinectin isoform	NULL		lacks	NULL					NULL	major portion of	kinesin-binding domain		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_32115_s_3	12773547	A kinectin isoform that lacks a major portion of the  kinesin-binding domain does not bind kinesin but interacts with another  resident of the endoplasmic reticulum, the translation elongation factor-1  delta (EF-1delta).	bind
47345	1	10650	5	13	NULL	NULL	NULL	Rabkinesin-6	GP		is a type of					kinesin-like protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_14_7933_s_190	10859366	A kinesin-like protein, termed Rabkinesin-6, has recently been identified that interacts with the GTP-bound forms of Rab6 ( 50).	bind
47346	2	10650	5	13	NULL	NULL	NULL	Rab6	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_14_7933_s_190	10859366	A kinesin-like protein, termed Rabkinesin-6, has recently been identified that interacts with the GTP-bound forms of Rab6 ( 50).	bind
47348	3	10650	5	13	NULL	NULL	NULL	Rabkinesin-6	GP		interacts with					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_14_7933_s_190	10859366	A kinesin-like protein, termed Rabkinesin-6, has recently been identified that interacts with the GTP-bound forms of Rab6 ( 50).	bind
39783	1	10650	6	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				Rab6	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_14_7933_s_190	10859366	A kinesin-like protein, termed Rabkinesin-6, has recently been identified that interacts with the GTP-bound forms of Rab6 ( 50).	bind
39784	2	10650	6	NULL	NULL	0	NULL	Rabkinesin-6	NULL		interacts with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_14_7933_s_190	10859366	A kinesin-like protein, termed Rabkinesin-6, has recently been identified that interacts with the GTP-bound forms of Rab6 ( 50).	bind
39785	3	10650	6	NULL	NULL	0	NULL	Rabkinesin-6	NULL		is a type of	NULL				kinesin-like protein	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_14_7933_s_190	10859366	A kinesin-like protein, termed Rabkinesin-6, has recently been identified that interacts with the GTP-bound forms of Rab6 ( 50).	bind
47379	1	10651	5	13	NULL	NULL	NULL	HNF-6	GP		bind									HNF-3beta site	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_22_13552_s_287	9593691	A kinetic analysis of HNF-6 binding to the HNF-3beta site showed that this difference results from a strong effect of linker length on the docking ( kon of HNF-6beta 60-fold higherR than that of HNF-6alpha) without much influence on the stability of the complex ( koff of HNF-6beta 3-fold higherR than that of HNF-6alpha).	bind
39954	1	10651	6	NULL	NULL	0	NULL	HNF-6	NULL		bind	NULL					NULL			HNF-3beta site	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_22_13552_s_287	9593691	A kinetic analysis of HNF-6 binding to the HNF-3beta site showed that this difference results from a strong effect of linker length on the docking ( kon of HNF-6beta 60-fold higherR than that of HNF-6alpha) without much influence on the stability of the complex ( koff of HNF-6beta 3-fold higherR than that of HNF-6alpha).	bind
47380	1	10652	5	13	NULL	NULL	NULL	siglec-2	GP	mouse	bind					Neu5Gc	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_12_8633_s_10	10722703	A known evolutionary difference is the strong preference of mouse siglec-2 (CD22) for Neu5Gc, contrasting with human siglec-2, which binds Neu5Ac equally well.	bind
47381	2	10652	5	13	NULL	NULL	NULL	siglec-2	GP	human	bind					Neu5Ac	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_12_8633_s_10	10722703	A known evolutionary difference is the strong preference of mouse siglec-2 (CD22) for Neu5Gc, contrasting with human siglec-2, which binds Neu5Ac equally well.	bind
47382	3	10652	5	13	NULL	NULL	NULL	statement 1	Process	affinity of	is equal to					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_12_8633_s_10	10722703	A known evolutionary difference is the strong preference of mouse siglec-2 (CD22) for Neu5Gc, contrasting with human siglec-2, which binds Neu5Ac equally well.	bind
47383	4	10652	5	13	NULL	NULL	NULL	statement 1	Process		is prefered over					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_12_8633_s_10	10722703	A known evolutionary difference is the strong preference of mouse siglec-2 (CD22) for Neu5Gc, contrasting with human siglec-2, which binds Neu5Ac equally well.	bind
47387	5	10652	5	13	NULL	NULL	NULL	CD22	GP		is 					siglec-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_12_8633_s_10	10722703	A known evolutionary difference is the strong preference of mouse siglec-2 (CD22) for Neu5Gc, contrasting with human siglec-2, which binds Neu5Ac equally well.	bind
39831	1	10652	6	NULL	NULL	0	NULL	siglec-2	NULL		is	NULL				CD22	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_12_8633_s_10	10722703	A known evolutionary difference is the strong preference of mouse siglec-2 (CD22) for Neu5Gc, contrasting with human siglec-2, which binds Neu5Ac equally well.	bind
39832	2	10652	6	NULL	NULL	0	NULL	siglec-2	NULL	mouse	bind	NULL				Neu5Gc	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_12_8633_s_10	10722703	A known evolutionary difference is the strong preference of mouse siglec-2 (CD22) for Neu5Gc, contrasting with human siglec-2, which binds Neu5Ac equally well.	bind
39833	3	10652	6	NULL	NULL	0	NULL	siglec-2	NULL	human	bind	NULL				Neu5Ac	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_12_8633_s_10	10722703	A known evolutionary difference is the strong preference of mouse siglec-2 (CD22) for Neu5Gc, contrasting with human siglec-2, which binds Neu5Ac equally well.	bind
39834	4	10652	6	NULL	NULL	0	NULL	statement 2	NULL	affinity of	is equal to	NULL				statement 3	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_12_8633_s_10	10722703	A known evolutionary difference is the strong preference of mouse siglec-2 (CD22) for Neu5Gc, contrasting with human siglec-2, which binds Neu5Ac equally well.	bind
50012	5	10652	6	10	NULL	0	NULL	statement 2	NULL		is preferred over	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_12_8633_s_10	10722703	A known evolutionary difference is the strong preference of mouse siglec-2 (CD22) for Neu5Gc, contrasting with human siglec-2, which binds Neu5Ac equally well.	bind
47386	1	10653	5	13	NULL	NULL	NULL	TBC 1269	Chemical		is a type of					L-selectin antagonist	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_microbesinfect_5_2_123_s_356	12650770	A known L-selectin antagonist, TBC 1269, not only inhibits RSV infectivity, but also inhibits annexin II-binding to its ligands, plasminogen and heparin indicating that the binding of annexin II to these three ligands is through a similar or closely associated site.	bind
47388	2	10653	5	13	NULL	NULL	NULL	TBC 1269	Chemical		inhibit					RSV 	Organism	infectivity of			NULL		NULL	NULL	NULL	NULL	gw60_microbesinfect_5_2_123_s_356	12650770	A known L-selectin antagonist, TBC 1269, not only inhibits RSV infectivity, but also inhibits annexin II-binding to its ligands, plasminogen and heparin indicating that the binding of annexin II to these three ligands is through a similar or closely associated site.	bind
47389	3	10653	5	13	NULL	NULL	NULL	annexin II	GP		bind					plasminogen	GP				NULL		NULL	NULL	NULL	NULL	gw60_microbesinfect_5_2_123_s_356	12650770	A known L-selectin antagonist, TBC 1269, not only inhibits RSV infectivity, but also inhibits annexin II-binding to its ligands, plasminogen and heparin indicating that the binding of annexin II to these three ligands is through a similar or closely associated site.	bind
47390	4	10653	5	13	NULL	NULL	NULL	annexin II	GP		bind					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_microbesinfect_5_2_123_s_356	12650770	A known L-selectin antagonist, TBC 1269, not only inhibits RSV infectivity, but also inhibits annexin II-binding to its ligands, plasminogen and heparin indicating that the binding of annexin II to these three ligands is through a similar or closely associated site.	bind
47391	5	10653	5	13	NULL	NULL	NULL	TBC 1269	Chemical		inhibit					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_microbesinfect_5_2_123_s_356	12650770	A known L-selectin antagonist, TBC 1269, not only inhibits RSV infectivity, but also inhibits annexin II-binding to its ligands, plasminogen and heparin indicating that the binding of annexin II to these three ligands is through a similar or closely associated site.	bind
47392	6	10653	5	13	NULL	NULL	NULL	TBC 1269	Chemical		inhibit					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_microbesinfect_5_2_123_s_356	12650770	A known L-selectin antagonist, TBC 1269, not only inhibits RSV infectivity, but also inhibits annexin II-binding to its ligands, plasminogen and heparin indicating that the binding of annexin II to these three ligands is through a similar or closely associated site.	bind
47396	7	10653	5	13	NULL	NULL	NULL	plasminogen	GP		is a type of					ligand	GP				NULL		NULL	NULL	NULL	NULL	gw60_microbesinfect_5_2_123_s_356	12650770	A known L-selectin antagonist, TBC 1269, not only inhibits RSV infectivity, but also inhibits annexin II-binding to its ligands, plasminogen and heparin indicating that the binding of annexin II to these three ligands is through a similar or closely associated site.	bind
47397	8	10653	5	13	NULL	NULL	NULL	heparin	Chemical		is a type of					ligand	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_microbesinfect_5_2_123_s_356	12650770	A known L-selectin antagonist, TBC 1269, not only inhibits RSV infectivity, but also inhibits annexin II-binding to its ligands, plasminogen and heparin indicating that the binding of annexin II to these three ligands is through a similar or closely associated site.	bind
39955	1	10653	6	NULL	NULL	0	NULL	TBC 1269	NULL		is a type of	NULL				L-selectin antagonist	NULL				NULL		0	NULL	NULL	NULL	gw60_microbesinfect_5_2_123_s_356	12650770	A known L-selectin antagonist, TBC 1269, not only inhibits RSV infectivity, but also inhibits annexin II-binding to its ligands, plasminogen and heparin indicating that the binding of annexin II to these three ligands is through a similar or closely associated site.	bind
39956	2	10653	6	10	NULL	0	NULL	TBC 1269			inhibits					RSV		infectivity of			NULL		NULL	NULL	NULL	NULL	gw60_microbesinfect_5_2_123_s_356	12650770	A known L-selectin antagonist, TBC 1269, not only inhibits RSV infectivity, but also inhibits annexin II-binding to its ligands, plasminogen and heparin indicating that the binding of annexin II to these three ligands is through a similar or closely associated site.	bind
39957	3	10653	6	NULL	NULL	0	NULL	annexin II	NULL		bind	NULL				plasminogen	NULL				NULL		0	NULL	NULL	NULL	gw60_microbesinfect_5_2_123_s_356	12650770	A known L-selectin antagonist, TBC 1269, not only inhibits RSV infectivity, but also inhibits annexin II-binding to its ligands, plasminogen and heparin indicating that the binding of annexin II to these three ligands is through a similar or closely associated site.	bind
39958	4	10653	6	NULL	NULL	0	NULL	annexin II	NULL		bind	NULL				heparin	NULL				NULL		0	NULL	NULL	NULL	gw60_microbesinfect_5_2_123_s_356	12650770	A known L-selectin antagonist, TBC 1269, not only inhibits RSV infectivity, but also inhibits annexin II-binding to its ligands, plasminogen and heparin indicating that the binding of annexin II to these three ligands is through a similar or closely associated site.	bind
39959	5	10653	6	NULL	NULL	0	NULL	TBC 1269	NULL		inhibits	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_microbesinfect_5_2_123_s_356	12650770	A known L-selectin antagonist, TBC 1269, not only inhibits RSV infectivity, but also inhibits annexin II-binding to its ligands, plasminogen and heparin indicating that the binding of annexin II to these three ligands is through a similar or closely associated site.	bind
39960	6	10653	6	NULL	NULL	0	NULL	TBC 1269	NULL		inhibits	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_microbesinfect_5_2_123_s_356	12650770	A known L-selectin antagonist, TBC 1269, not only inhibits RSV infectivity, but also inhibits annexin II-binding to its ligands, plasminogen and heparin indicating that the binding of annexin II to these three ligands is through a similar or closely associated site.	bind
47398	1	10654	5	13	NULL	NULL	NULL	KRAB-ZFP	GP		bind		sequence specifically	C2H2 zinc fingers		DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_24_18000_s_383	10748030	A KRAB-ZFP binds target gene DNA sequence-specifically through its array of C2H2 zinc fingers.	bind
39835	1	10654	6	NULL	NULL	0	NULL	KRAB-ZFP	NULL		bind	NULL	sequence specifically	C2H2 zinc fingers		DNA 	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_24_18000_s_383	10748030	A KRAB-ZFP binds target gene DNA sequence-specifically through its array of C2H2 zinc fingers.	bind
47399	1	10655	5	13	NULL	NULL	NULL	I-RNA	NucleicAcid	yeast	bind		strongly			La antigen	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_36_27531_s_340	10856291	A La depletion/add-back approach was also employed by Das  et al. ( 50) during their studies on the inhibition of the HCV IRES-mediated translation by yeast I-RNA, which strongly binds human La antigen.	bind
47400	2	10655	5	13	NULL	NULL	NULL	IRES	NucleicAcid		mediates					HCV	Organism	translation of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_36_27531_s_340	10856291	A La depletion/add-back approach was also employed by Das  et al. ( 50) during their studies on the inhibition of the HCV IRES-mediated translation by yeast I-RNA, which strongly binds human La antigen.	bind
47401	3	10655	5	13	NULL	NULL	NULL	I-RNA	NucleicAcid	yeast	inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_36_27531_s_340	10856291	A La depletion/add-back approach was also employed by Das  et al. ( 50) during their studies on the inhibition of the HCV IRES-mediated translation by yeast I-RNA, which strongly binds human La antigen.	bind
39836	1	10655	6	NULL	NULL	0	NULL	I-RNA	NULL	yeast	bind	NULL	strongly			La antigen	NULL	human			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_36_27531_s_340	10856291	A La depletion/add-back approach was also employed by Das  et al. ( 50) during their studies on the inhibition of the HCV IRES-mediated translation by yeast I-RNA, which strongly binds human La antigen.	bind
39837	2	10655	6	NULL	NULL	0	NULL	IRES	NULL		mediates	NULL				HCV	NULL	translation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_36_27531_s_340	10856291	A La depletion/add-back approach was also employed by Das  et al. ( 50) during their studies on the inhibition of the HCV IRES-mediated translation by yeast I-RNA, which strongly binds human La antigen.	bind
39838	3	10655	6	NULL	NULL	0	NULL	I-RNA	NULL	yeast	inhibits	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_36_27531_s_340	10856291	A La depletion/add-back approach was also employed by Das  et al. ( 50) during their studies on the inhibition of the HCV IRES-mediated translation by yeast I-RNA, which strongly binds human La antigen.	bind
47402	1	10656	5	13	NULL	NULL	NULL	Ad5 origin fragment	NucleicAcid	labeled	bind					GST-POU	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_6_3398_s_164	9013582	A labeled Ad5 origin fragment bound by GST-POU was immobilized on GA beads (Fig.  5 A).	bind
39839	1	10656	6	NULL	NULL	0	NULL	Ad5 origin fragment	NULL		bind	NULL				GST-POU	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_6_3398_s_164	9013582	A labeled Ad5 origin fragment bound by GST-POU was immobilized on GA beads (Fig.  5 A).	bind
47403	1	10657	5	13	NULL	NULL	NULL	oligonucleotide	NucleicAcid	mutant;;labeled	does not bind				PU.1 site (P106M)	PU.1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_13_9098_s_199	10085160	A labeled oligonucleotide mutated at the PU.1 site (P106M) did not bind PU.1 ( lane 8) and a labeled Sp1 mutant (S91M) did not bind Sp1 ( lane 9).	bind
47404	2	10657	5	13	NULL	NULL	NULL	Sp1	GP	mutant;;labeled	does not bind			S91M		Sp1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_13_9098_s_199	10085160	A labeled oligonucleotide mutated at the PU.1 site (P106M) did not bind PU.1 ( lane 8) and a labeled Sp1 mutant (S91M) did not bind Sp1 ( lane 9).	bind
39840	1	10657	6	NULL	NULL	0	NULL	oligonucleotide	NULL	mutant	does not bind	NULL			PU.1 site (P106M)	PU.1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_13_9098_s_199	10085160	A labeled oligonucleotide mutated at the PU.1 site (P106M) did not bind PU.1 ( lane 8) and a labeled Sp1 mutant (S91M) did not bind Sp1 ( lane 9).	bind
39841	2	10657	6	10	NULL	0	NULL	Sp1	NULL	mutant;;labeled	does not bind	NULL		S91M		Sp1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_13_9098_s_199	10085160	A labeled oligonucleotide mutated at the PU.1 site (P106M) did not bind PU.1 ( lane 8) and a labeled Sp1 mutant (S91M) did not bind Sp1 ( lane 9).	bind
47405	1	10659	5	13	NULL	NULL	NULL	Hu HB-EGF	GP	recombinant;;mature	is identical to			63 to 148		HB-EGF	GP	mature;;monkey			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2344_s_51	11953369	A laboratory earlier reported that recombinant mature Hu HB-EGF (residues 63 to 148), which is identical to the mature Mk HB-EGF (except that Asn87 of human is replaced with Ser87 in the monkey [Fig.  1]), strongly inhibits the binding of radiolabeled DT to toxin receptor-bearing cells ( 26).	bind
47406	2	10659	5	13	NULL	NULL	NULL	cells	Cell		bear					toxin receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2344_s_51	11953369	A laboratory earlier reported that recombinant mature Hu HB-EGF (residues 63 to 148), which is identical to the mature Mk HB-EGF (except that Asn87 of human is replaced with Ser87 in the monkey [Fig.  1]), strongly inhibits the binding of radiolabeled DT to toxin receptor-bearing cells ( 26).	bind
47407	3	10659	5	13	NULL	NULL	NULL	DT	GP	radiolabeled	bind					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2344_s_51	11953369	A laboratory earlier reported that recombinant mature Hu HB-EGF (residues 63 to 148), which is identical to the mature Mk HB-EGF (except that Asn87 of human is replaced with Ser87 in the monkey [Fig.  1]), strongly inhibits the binding of radiolabeled DT to toxin receptor-bearing cells ( 26).	bind
47408	4	10659	5	13	NULL	NULL	NULL	statement 1	Process		inhibit		strongly			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2344_s_51	11953369	A laboratory earlier reported that recombinant mature Hu HB-EGF (residues 63 to 148), which is identical to the mature Mk HB-EGF (except that Asn87 of human is replaced with Ser87 in the monkey [Fig.  1]), strongly inhibits the binding of radiolabeled DT to toxin receptor-bearing cells ( 26).	bind
39971	1	10659	6	NULL	NULL	0	NULL	DT	NULL	radiolabeled	bind	NULL				toxin receptor-bearing cells	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_5_2344_s_51	11953369	A laboratory earlier reported that recombinant mature Hu HB-EGF (residues 63 to 148), which is identical to the mature Mk HB-EGF (except that Asn87 of human is replaced with Ser87 in the monkey [Fig.  1]), strongly inhibits the binding of radiolabeled DT to toxin receptor-bearing cells ( 26).	bind
39973	2	10659	6	NULL	NULL	0	NULL	HB-EGF	NULL	recombinant;; mature;; human	inhibits	NULL	strongly	residues 63 to 148		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2344_s_51	11953369	A laboratory earlier reported that recombinant mature Hu HB-EGF (residues 63 to 148), which is identical to the mature Mk HB-EGF (except that Asn87 of human is replaced with Ser87 in the monkey [Fig.  1]), strongly inhibits the binding of radiolabeled DT to toxin receptor-bearing cells ( 26).	bind
39974	3	10659	6	NULL	NULL	0	NULL	HB-EGF	NULL	recombinant;; mature;; human	is identical to	NULL				HB-EGF	NULL	mature;; monkey			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2344_s_51	11953369	A laboratory earlier reported that recombinant mature Hu HB-EGF (residues 63 to 148), which is identical to the mature Mk HB-EGF (except that Asn87 of human is replaced with Ser87 in the monkey [Fig.  1]), strongly inhibits the binding of radiolabeled DT to toxin receptor-bearing cells ( 26).	bind
47409	1	10661	5	13	NULL	NULL	NULL	ephedrine	Chemical		bind					beta3-adrenoreceptors	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_clin-sci-(lond)_96_5_10209080_s_11	10209080	A lack  of binding of ephedrine to beta3-adrenoreceptors and the observed decrease  in urinary noradrenaline during ephedrine treatment suggest that the thermogenic  effect of ephedrine results from direct beta1-/beta2-adrenoreceptor agonism.	bind
47410	2	10661	5	13	NULL	NULL	NULL	statement 1	Process		occurs during					ephedrine	Chemical	treatment			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_clin-sci-(lond)_96_5_10209080_s_11	10209080	A lack  of binding of ephedrine to beta3-adrenoreceptors and the observed decrease  in urinary noradrenaline during ephedrine treatment suggest that the thermogenic  effect of ephedrine results from direct beta1-/beta2-adrenoreceptor agonism.	bind
47411	3	10661	5	13	NULL	NULL	NULL	ephedrine	Chemical	treatment with	decreases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_clin-sci-(lond)_96_5_10209080_s_11	10209080	A lack  of binding of ephedrine to beta3-adrenoreceptors and the observed decrease  in urinary noradrenaline during ephedrine treatment suggest that the thermogenic  effect of ephedrine results from direct beta1-/beta2-adrenoreceptor agonism.	bind
47412	4	10661	5	13	NULL	NULL	NULL	ephedrine	Chemical		possess					thermogenic effect					NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_clin-sci-(lond)_96_5_10209080_s_11	10209080	A lack  of binding of ephedrine to beta3-adrenoreceptors and the observed decrease  in urinary noradrenaline during ephedrine treatment suggest that the thermogenic  effect of ephedrine results from direct beta1-/beta2-adrenoreceptor agonism.	bind
47413	5	10661	5	13	NULL	NULL	NULL	statement 4	Process		results from					beta1-/beta2-adrenoreceptor agonism	Process	direct			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_clin-sci-(lond)_96_5_10209080_s_11	10209080	A lack  of binding of ephedrine to beta3-adrenoreceptors and the observed decrease  in urinary noradrenaline during ephedrine treatment suggest that the thermogenic  effect of ephedrine results from direct beta1-/beta2-adrenoreceptor agonism.	bind
39975	1	10661	6	NULL	NULL	0	NULL	ephedrine	NULL		bind	NULL				beta3-adrenoreceptors	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_clin-sci-(lond)_96_5_10209080_s_11	10209080	A lack  of binding of ephedrine to beta3-adrenoreceptors and the observed decrease  in urinary noradrenaline during ephedrine treatment suggest that the thermogenic  effect of ephedrine results from direct beta1-/beta2-adrenoreceptor agonism.	bind
39976	2	10661	6	NULL	NULL	0	NULL	ephedrine	NULL	treatment with	decreases	NULL				noradrenaline 	NULL	urinary			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_clin-sci-(lond)_96_5_10209080_s_11	10209080	A lack  of binding of ephedrine to beta3-adrenoreceptors and the observed decrease  in urinary noradrenaline during ephedrine treatment suggest that the thermogenic  effect of ephedrine results from direct beta1-/beta2-adrenoreceptor agonism.	bind
39977	3	10661	6	NULL	NULL	0	NULL	ephedrine	NULL	treatment with	decreases	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_clin-sci-(lond)_96_5_10209080_s_11	10209080	A lack  of binding of ephedrine to beta3-adrenoreceptors and the observed decrease  in urinary noradrenaline during ephedrine treatment suggest that the thermogenic  effect of ephedrine results from direct beta1-/beta2-adrenoreceptor agonism.	bind
39980	4	10661	6	10	NULL	0	NULL	ephedrine	NULL		possess	NULL				thermogenic effect	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_clin-sci-(lond)_96_5_10209080_s_11	10209080	A lack  of binding of ephedrine to beta3-adrenoreceptors and the observed decrease  in urinary noradrenaline during ephedrine treatment suggest that the thermogenic  effect of ephedrine results from direct beta1-/beta2-adrenoreceptor agonism.	bind
39981	5	10661	6	NULL	NULL	0	NULL	statement 4	NULL		results from	NULL				beta1-/beta2-adrenoreceptor agonism	NULL	direct			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_clin-sci-(lond)_96_5_10209080_s_11	10209080	A lack  of binding of ephedrine to beta3-adrenoreceptors and the observed decrease  in urinary noradrenaline during ephedrine treatment suggest that the thermogenic  effect of ephedrine results from direct beta1-/beta2-adrenoreceptor agonism.	bind
47416	1	10662	5	13	NULL	NULL	NULL	Mgat3 T37 gene	GP		express					GlcNAc-TIII activity	GP				NULL	LEC10 CHO cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_29_26300_s_228	11986323	A lack of a dominant-negative effect was confirmed by overexpressing a cDNA encoding the  Mgat3 T37 gene in LEC10 CHO cells, which express GlcNAc-TIII activity ( 3), due to a gain-of-function mutation that activates transcription of the endogenous  Mgat3 gene.	bind
47418	2	10662	5	13	NULL	NULL	NULL	function mutation	Process		activates					Mgat3 gene	GP	transcription of;;endogenous			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_29_26300_s_228	11986323	A lack of a dominant-negative effect was confirmed by overexpressing a cDNA encoding the  Mgat3 T37 gene in LEC10 CHO cells, which express GlcNAc-TIII activity ( 3), due to a gain-of-function mutation that activates transcription of the endogenous  Mgat3 gene.	bind
39982	1	10662	6	10	NULL	0	NULL	Mgat3 T37 gene	NULL		express	NULL				GlcNAc-TIII activity	NULL				NULL	LEC10 CHO cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_29_26300_s_228	11986323	A lack of a dominant-negative effect was confirmed by overexpressing a cDNA encoding the  Mgat3 T37 gene in LEC10 CHO cells, which express GlcNAc-TIII activity ( 3), due to a gain-of-function mutation that activates transcription of the endogenous  Mgat3 gene.	bind
50248	2	10662	6	10	NULL	0	NULL	function mutation	NULL		activates	NULL				Mgat3 gene	NULL	transcription of;; endogenous 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26300_s_228	11986323	A lack of a dominant-negative effect was confirmed by overexpressing a cDNA encoding the  Mgat3 T37 gene in LEC10 CHO cells, which express GlcNAc-TIII activity ( 3), due to a gain-of-function mutation that activates transcription of the endogenous  Mgat3 gene.	bind
47420	1	10663	5	13	NULL	NULL	NULL	actophorin	GP		does not bind					ADP-Pi filaments	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_22_15538_s_307	10336448	A lack of actophorin binding to ADP-Pi filaments and phalloidin-ADP filaments in pelleting assays establishes that the absence of a fluorescence signal is due to a lack of binding rather than failure of bound actophorin to induce a fluorescence change in pyrenyl ADP-Pi-actin filaments.	bind
47421	2	10663	5	13	NULL	NULL	NULL	actophorin	GP		does not bind					phalloidin-ADP filaments	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_22_15538_s_307	10336448	A lack of actophorin binding to ADP-Pi filaments and phalloidin-ADP filaments in pelleting assays establishes that the absence of a fluorescence signal is due to a lack of binding rather than failure of bound actophorin to induce a fluorescence change in pyrenyl ADP-Pi-actin filaments.	bind
39842	1	10663	6	NULL	NULL	0	NULL	actophorin	NULL		does not bind	NULL				ADP-pi filaments	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_22_15538_s_307	10336448	A lack of actophorin binding to ADP-Pi filaments and phalloidin-ADP filaments in pelleting assays establishes that the absence of a fluorescence signal is due to a lack of binding rather than failure of bound actophorin to induce a fluorescence change in pyrenyl ADP-Pi-actin filaments.	bind
39843	2	10663	6	NULL	NULL	0	NULL	actophorin	NULL		does not bind	NULL				phalloidin-ADP filaments	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_22_15538_s_307	10336448	A lack of actophorin binding to ADP-Pi filaments and phalloidin-ADP filaments in pelleting assays establishes that the absence of a fluorescence signal is due to a lack of binding rather than failure of bound actophorin to induce a fluorescence change in pyrenyl ADP-Pi-actin filaments.	bind
47423	1	10665	5	13	NULL	NULL	NULL	Sec9p/Sso1p	GP		bind					v-SNARE Sec22p	GP	ER-Golgi			NULL		NULL	NULL	NULL	NULL	gw60_genetics_155_4_1643_s_163	10924463	A lack of specificity is seen in formation of the ternary complex, however, as Sec9p/Sso1p will bind to the ER-Golgi v-SNARE Sec22p ( D ASCHER et al. 1991   ;	bind
39997	1	10665	6	10	NULL	0	NULL	Sec9p/Sso1p	NULL		bind	NULL				v-SNARE Sec22p	NULL	ER-Golgi 			NULL		NULL	NULL	NULL	NULL	gw60_genetics_155_4_1643_s_163	10924463	A lack of specificity is seen in formation of the ternary complex, however, as Sec9p/Sso1p will bind to the ER-Golgi v-SNARE Sec22p ( D ASCHER et al. 1991   ;	bind
47424	1	10666	5	13	NULL	NULL	NULL	laminin	GP		bind					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-biol-chem_267_25_1387642_s_2	1387642	A laminin-binding peptide (peptide G), predicted from the cDNA sequence  for a 33-kDa protein related to the 67-kDa laminin receptor, specifically  inhibits binding of laminin to heparin and sulfatide.	bind
47425	2	10666	5	13	NULL	NULL	NULL	laminin	GP		bind					sulfatide	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-biol-chem_267_25_1387642_s_2	1387642	A laminin-binding peptide (peptide G), predicted from the cDNA sequence  for a 33-kDa protein related to the 67-kDa laminin receptor, specifically  inhibits binding of laminin to heparin and sulfatide.	bind
47426	3	10666	5	13	NULL	NULL	NULL	laminin-binding peptide	GP		inhibit		specifically			statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-biol-chem_267_25_1387642_s_2	1387642	A laminin-binding peptide (peptide G), predicted from the cDNA sequence  for a 33-kDa protein related to the 67-kDa laminin receptor, specifically  inhibits binding of laminin to heparin and sulfatide.	bind
47427	4	10666	5	13	NULL	NULL	NULL	laminin-binding peptide	GP		inhibit		specifically			statement 2	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-biol-chem_267_25_1387642_s_2	1387642	A laminin-binding peptide (peptide G), predicted from the cDNA sequence  for a 33-kDa protein related to the 67-kDa laminin receptor, specifically  inhibits binding of laminin to heparin and sulfatide.	bind
50249	5	10666	5	13	NULL	NULL	NULL	peptide G	GP		is a type of					 laminin-binding peptide	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-biol-chem_267_25_1387642_s_2	1387642	A laminin-binding peptide (peptide G), predicted from the cDNA sequence  for a 33-kDa protein related to the 67-kDa laminin receptor, specifically  inhibits binding of laminin to heparin and sulfatide.	bind
40000	1	10666	6	NULL	NULL	0	NULL	laminin	NULL		bind	NULL				heparin	NULL				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_j-biol-chem_267_25_1387642_s_2	1387642	A laminin-binding peptide (peptide G), predicted from the cDNA sequence  for a 33-kDa protein related to the 67-kDa laminin receptor, specifically  inhibits binding of laminin to heparin and sulfatide.	bind
40001	2	10666	6	NULL	NULL	0	NULL	laminin	NULL		bind	NULL				sulfatide	NULL				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_j-biol-chem_267_25_1387642_s_2	1387642	A laminin-binding peptide (peptide G), predicted from the cDNA sequence  for a 33-kDa protein related to the 67-kDa laminin receptor, specifically  inhibits binding of laminin to heparin and sulfatide.	bind
40002	3	10666	6	10	NULL	0	NULL	laminin-binding peptide 	NULL		inhibits	NULL	specifically			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-biol-chem_267_25_1387642_s_2	1387642	A laminin-binding peptide (peptide G), predicted from the cDNA sequence  for a 33-kDa protein related to the 67-kDa laminin receptor, specifically  inhibits binding of laminin to heparin and sulfatide.	bind
40003	4	10666	6	10	NULL	0	NULL	laminin-binding peptide 	NULL		inhibits	NULL	specifically			statement 2	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-biol-chem_267_25_1387642_s_2	1387642	A laminin-binding peptide (peptide G), predicted from the cDNA sequence  for a 33-kDa protein related to the 67-kDa laminin receptor, specifically  inhibits binding of laminin to heparin and sulfatide.	bind
50250	5	10666	6	10	NULL	0	NULL	peptide G	NULL		is a type of	NULL				 laminin-binding peptide	NULL				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_j-biol-chem_267_25_1387642_s_2	1387642	A laminin-binding peptide (peptide G), predicted from the cDNA sequence  for a 33-kDa protein related to the 67-kDa laminin receptor, specifically  inhibits binding of laminin to heparin and sulfatide.	bind
47428	1	10667	5	13	NULL	NULL	NULL	ADAMTS4	GP	125I-labeled	bind					fibronectin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_31_32483_s_146	15161923	A large amount of 125I-labeled ADAMTS4 could bind to intact fibronectin-coated wells, whereas BSA-coated wells showed only back-ground binding.	bind
40007	1	10667	6	10	NULL	0	NULL	ADAMTS4		125I-labeled	bind					fibronectin					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_31_32483_s_146	15161923	A large amount of 125I-labeled ADAMTS4 could bind to intact fibronectin-coated wells, whereas BSA-coated wells showed only back-ground binding.	bind
47429	1	10668	5	13	NULL	NULL	NULL	IP(3)	Chemical		is					1,4,5-trisphosphate	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0580-0599_biophys-j_89_2_15908571_s_2	15908571	A large amount of data and observations on inositol 1,4,5-trisphosphate  (IP(3)) binding to the IP(3) receptor/Ca(2+) channel, the steady-state  activity of the channel, and its inactivation by IP(3) can be explained  by assuming one activation and one inhibition module, both allosterically  operated by Ca(2+), IP(3), and ATP, and one adaptation element, driven  by IP(3), Ca(2+), and the interconversion between two possible conformations  of the receptor.	bind
47430	2	10668	5	13	NULL	NULL	NULL	IP(3)	Chemical		bind					IP(3) receptor/Ca(2+) channel	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0580-0599_biophys-j_89_2_15908571_s_2	15908571	A large amount of data and observations on inositol 1,4,5-trisphosphate  (IP(3)) binding to the IP(3) receptor/Ca(2+) channel, the steady-state  activity of the channel, and its inactivation by IP(3) can be explained  by assuming one activation and one inhibition module, both allosterically  operated by Ca(2+), IP(3), and ATP, and one adaptation element, driven  by IP(3), Ca(2+), and the interconversion between two possible conformations  of the receptor.	bind
47431	3	10668	5	13	NULL	NULL	NULL	IP(3)	Chemical		inactivates					IP(3) receptor/Ca(2+) channel	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0580-0599_biophys-j_89_2_15908571_s_2	15908571	A large amount of data and observations on inositol 1,4,5-trisphosphate  (IP(3)) binding to the IP(3) receptor/Ca(2+) channel, the steady-state  activity of the channel, and its inactivation by IP(3) can be explained  by assuming one activation and one inhibition module, both allosterically  operated by Ca(2+), IP(3), and ATP, and one adaptation element, driven  by IP(3), Ca(2+), and the interconversion between two possible conformations  of the receptor.	bind
40399	1	10668	6	NULL	NULL	0	NULL	IP(3)	NULL		is	NULL				inositol 1,4,5-trisphosphate	NULL				NULL		0	NULL	NULL	NULL	abs-batch0580-0599_biophys-j_89_2_15908571_s_2	15908571	A large amount of data and observations on inositol 1,4,5-trisphosphate  (IP(3)) binding to the IP(3) receptor/Ca(2+) channel, the steady-state  activity of the channel, and its inactivation by IP(3) can be explained  by assuming one activation and one inhibition module, both allosterically  operated by Ca(2+), IP(3), and ATP, and one adaptation element, driven  by IP(3), Ca(2+), and the interconversion between two possible conformations  of the receptor.	bind
40400	2	10668	6	NULL	NULL	0	NULL	IP(3)	NULL		bind	NULL				IP(3) receptor/Ca(2+) channel	NULL				NULL		0	NULL	NULL	NULL	abs-batch0580-0599_biophys-j_89_2_15908571_s_2	15908571	A large amount of data and observations on inositol 1,4,5-trisphosphate  (IP(3)) binding to the IP(3) receptor/Ca(2+) channel, the steady-state  activity of the channel, and its inactivation by IP(3) can be explained  by assuming one activation and one inhibition module, both allosterically  operated by Ca(2+), IP(3), and ATP, and one adaptation element, driven  by IP(3), Ca(2+), and the interconversion between two possible conformations  of the receptor.	bind
40418	3	10668	6	NULL	NULL	0	NULL	IP(3)	NULL		inactivates	NULL				IP(3) receptor/Ca(2+) channel	NULL				NULL		0	NULL	NULL	NULL	abs-batch0580-0599_biophys-j_89_2_15908571_s_2	15908571	A large amount of data and observations on inositol 1,4,5-trisphosphate  (IP(3)) binding to the IP(3) receptor/Ca(2+) channel, the steady-state  activity of the channel, and its inactivation by IP(3) can be explained  by assuming one activation and one inhibition module, both allosterically  operated by Ca(2+), IP(3), and ATP, and one adaptation element, driven  by IP(3), Ca(2+), and the interconversion between two possible conformations  of the receptor.	bind
47432	1	10669	5	13	NULL	NULL	NULL	phosphate	Chemical		bind					L. casei TS	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-mol-biol_232_4_8371269_s_15	8371269	A large and a small P6(1)22 crystal form are observed for  both phosphate-bound and dUMP-bound L. casei TS.	bind
47433	2	10669	5	13	NULL	NULL	NULL	dUMP	Chemical		bind					L. casei TS	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-mol-biol_232_4_8371269_s_15	8371269	A large and a small P6(1)22 crystal form are observed for  both phosphate-bound and dUMP-bound L. casei TS.	bind
40012	1	10669	6	NULL	NULL	0	NULL	L. casei TS	NULL		bind	NULL				dUMP	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-mol-biol_232_4_8371269_s_15	8371269	A large and a small P6(1)22 crystal form are observed for  both phosphate-bound and dUMP-bound L. casei TS.	bind
40013	2	10669	6	NULL	NULL	0	NULL	L. casei TS	NULL		bind	NULL				phosphate	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-mol-biol_232_4_8371269_s_15	8371269	A large and a small P6(1)22 crystal form are observed for  both phosphate-bound and dUMP-bound L. casei TS.	bind
47434	1	10670	5	13	NULL	NULL	NULL	rhodopsin	GP		bind					arrestin	GP	visual			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_14_11703_s_180	11809770	A large conformational change has been suggested to occur when rhodopsin binds to visual arrestin, which could assemble many recognition elements to create a continuous receptor-binding surface ( 44).	bind
47435	2	10670	5	13	NULL	NULL	NULL	statement 1	GP		assemble					recognition elements	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_14_11703_s_180	11809770	A large conformational change has been suggested to occur when rhodopsin binds to visual arrestin, which could assemble many recognition elements to create a continuous receptor-binding surface ( 44).	bind
47436	3	10670	5	13	NULL	NULL	NULL	statement 2	Process		creates					receptor-binding surface	GP	continuous			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_14_11703_s_180	11809770	A large conformational change has been suggested to occur when rhodopsin binds to visual arrestin, which could assemble many recognition elements to create a continuous receptor-binding surface ( 44).	bind
40014	1	10670	6	NULL	NULL	0	NULL	rhodopsin	NULL		bind	NULL				arrestin	NULL	visual			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_14_11703_s_180	11809770	A large conformational change has been suggested to occur when rhodopsin binds to visual arrestin, which could assemble many recognition elements to create a continuous receptor-binding surface ( 44).	bind
40045	2	10670	6	NULL	NULL	0	NULL	statement 1	NULL		creates	NULL				conformational change	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_14_11703_s_180	11809770	A large conformational change has been suggested to occur when rhodopsin binds to visual arrestin, which could assemble many recognition elements to create a continuous receptor-binding surface ( 44).	bind
40046	3	10670	6	NULL	NULL	0	NULL	statement 2	NULL		creates	NULL				receptor-binding surface	NULL	continuous			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_14_11703_s_180	11809770	A large conformational change has been suggested to occur when rhodopsin binds to visual arrestin, which could assemble many recognition elements to create a continuous receptor-binding surface ( 44).	bind
40047	4	10670	6	NULL	NULL	0	NULL	statement 3	NULL		occurs via	NULL				recognition elements	NULL	assembly of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_14_11703_s_180	11809770	A large conformational change has been suggested to occur when rhodopsin binds to visual arrestin, which could assemble many recognition elements to create a continuous receptor-binding surface ( 44).	bind
47437	1	10671	5	13	NULL	NULL	NULL	Lin bone marrow cells	Cell		bind		specifically			Fc-FGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_4_2_241_s_44	12586067	A large fraction of Lin  bone marrow cells specifically binds the Fc-FGF fusion protein (B).	bind
47438	2	10671	5	13	NULL	NULL	NULL	Fc-FGF	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_4_2_241_s_44	12586067	A large fraction of Lin  bone marrow cells specifically binds the Fc-FGF fusion protein (B).	bind
40048	1	10671	6	10	NULL	0	NULL	Lin bone marrow cells	NULL		bind	NULL	specifically			Fc-FGF 	NULL				NULL		NULL	NULL	NULL	NULL	gw60_devcell_4_2_241_s_44	12586067	A large fraction of Lin  bone marrow cells specifically binds the Fc-FGF fusion protein (B).	bind
50251	2	10671	6	10	NULL	0	NULL	Fc-FGF	NULL		is a type of	NULL				fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw60_devcell_4_2_241_s_44	12586067	A large fraction of Lin  bone marrow cells specifically binds the Fc-FGF fusion protein (B).	bind
47439	1	10672	5	13	NULL	NULL	NULL	DNA ligase IIIalpha	GP	mitochondrial	does not bind					XRCC1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_52_48978_s_258	11598119	A large fraction of the mtDNA ligase IIIalpha did not bind the XRCC1 column, suggesting that it may be associated with a protein that blocks this interaction.	bind
40050	1	10672	6	10	NULL	0	NULL	DNA ligase IIIalpha	NULL	mitochondrial 	does not bind	NULL				XRCC1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_52_48978_s_258	11598119	A large fraction of the mtDNA ligase IIIalpha did not bind the XRCC1 column, suggesting that it may be associated with a protein that blocks this interaction.	bind
48019	1	10673	5	13	NULL	NULL	NULL	8A6	GP		interacts with					CD36	GP		immunodominant domain (aa 155-183)		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
48020	2	10673	5	13	NULL	NULL	NULL	statement 1	Process		blocks					CD36	GP	function of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
48021	3	10673	5	13	NULL	NULL	NULL	CD36 	GP		function in					TSP	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
50765	4	10673	5	13	NULL	NULL	NULL	CD36	GP		function in					collagen	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
50766	5	10673	5	13	NULL	NULL	NULL	CD36	GP		function in					malaria	MedicalFinding	cytoadhesion of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
50767	6	10673	5	13	NULL	NULL	NULL	CD36	GP		function in					apoptotic cells	Cell	uptake of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
50768	7	10673	5	13	NULL	NULL	NULL	CD36	GP		function in					Ox-LDL	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
50769	8	10673	5	13	NULL	NULL	NULL	8A6	GP		is a type of					\tmonoclonal antibody against human CD36	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
50770	9	10673	5	13	NULL	NULL	NULL	OKM5	GP		is a type of					monoclonal antibody against human CD36	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
50771	10	10673	5	13	NULL	NULL	NULL	FA6-152	GP		is a type of					\tmonoclonal antibody against human CD36	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
50772	11	10673	5	13	NULL	NULL	NULL	L103	GP		is a type of					monoclonal antibody against human CD36	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
50773	12	10673	5	13	NULL	NULL	NULL	5F1	GP		is a type of					monoclonal antibody against human CD36	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
50774	13	10673	5	13	NULL	NULL	NULL	Smphi	GP		is a type of					monoclonal antibody against human CD36	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
50775	14	10673	5	13	NULL	NULL	NULL	ESIVC7	GP		is a type of					monoclonal antibody against human CD36	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
50776	15	10673	5	13	NULL	NULL	NULL	10/5	GP		is a type of					monoclonal antibody against human CD36	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
50777	16	10673	5	13	NULL	NULL	NULL	OKM5	GP		interacts with					CD36	GP		\timmunodominant domain (aa 155-183)		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
50778	17	10673	5	13	NULL	NULL	NULL	statement 16	Process		blocks					CD36	GP	function of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
50779	18	10673	5	13	NULL	NULL	NULL	FA6-152	GP		interacts with					CD36	GP		immunodominant domain (aa 155-183)		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
50780	19	10673	5	13	NULL	NULL	NULL	statement 18	Process		blocks					CD36	GP	function of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
50781	20	10673	5	13	NULL	NULL	NULL	L103	GP		interacts with					CD36	GP		immunodominant domain (aa 155-183)		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
50782	21	10673	5	13	NULL	NULL	NULL	statement 20	Process		blocks					CD36	GP	function of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
50783	22	10673	5	13	NULL	NULL	NULL	5F1	GP		interacts with					CD36	GP		immunodominant domain (aa 155-183)		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
50784	23	10673	5	13	NULL	NULL	NULL	statement 22	Process		blocks					CD36	GP	function of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
50785	24	10673	5	13	NULL	NULL	NULL	Smphi	GP		interacts with					CD36	GP		immunodominant domain (aa 155-183)		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
50786	25	10673	5	13	NULL	NULL	NULL	statement 24	Process		blocks					CD36	GP	function of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
50787	26	10673	5	13	NULL	NULL	NULL	ESIVC7	GP		interacts with					CD36	GP		immunodominant domain (aa 155-183)		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
50788	27	10673	5	13	NULL	NULL	NULL	statement 26	Process		blocks					CD36	GP	function of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
50789	28	10673	5	13	NULL	NULL	NULL	10/5	GP		interacts with					CD36	GP		immunodominant domain (aa 155-183)		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
50790	29	10673	5	13	NULL	NULL	NULL	statement 28	Process		blocks					CD36	GP	function of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
50791	30	10673	5	13	NULL	NULL	NULL	CD36	GP		function in					ROS	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
40419	1	10673	6	NULL	NULL	0	NULL	CD36	NULL		function in	NULL				TSP	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
40420	2	10673	6	NULL	NULL	0	NULL	CD36	NULL		functions in	NULL				collagen	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
40421	3	10673	6	NULL	NULL	0	NULL	CD36	NULL		functions in	NULL				malaria	NULL	cytoadhesion of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
40422	4	10673	6	NULL	NULL	0	NULL	CD36	NULL		functions in	NULL				apoptotic cells	NULL	uptake of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
40423	5	10673	6	NULL	NULL	0	NULL	CD36	NULL		functions in	NULL				ROS	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
40424	6	10673	6	NULL	NULL	0	NULL	CD36	NULL		functions in	NULL				Ox-LDL	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
40425	7	10673	6	NULL	NULL	0	NULL	8A6	NULL		is a type of	NULL				monoclonal antibody against human CD36	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
40426	8	10673	6	NULL	NULL	0	NULL	OKM5	NULL		is a type of	NULL				monoclonal antibody against human CD36	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
40427	9	10673	6	NULL	NULL	0	NULL	FA6-152	NULL		is a type of	NULL				monoclonal antibody against human CD36	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
40428	10	10673	6	NULL	NULL	0	NULL	L103	NULL		is a type of	NULL				monoclonal antibody against human CD36	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
40429	11	10673	6	NULL	NULL	0	NULL	5F1	NULL		is a type of	NULL				monoclonal antibody against human CD36	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
40430	12	10673	6	NULL	NULL	0	NULL	Smphi	NULL		is a type of	NULL				monoclonal antibody against human CD36	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
40431	13	10673	6	NULL	NULL	0	NULL	ESIVC7	NULL		is a type of	NULL				monoclonal antibody against human CD36	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
40432	14	10673	6	NULL	NULL	0	NULL	10/5	NULL		is a type of	NULL				monoclonal antibody against human CD36	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
40433	15	10673	6	NULL	NULL	0	NULL	8A6	NULL		interacts with	NULL				CD36	NULL		immunodominant domain (aa 155-183)		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
40437	16	10673	6	NULL	NULL	0	NULL	statement 15	NULL		blocks	NULL				CD36	NULL	function of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
40438	17	10673	6	NULL	NULL	0	NULL	OKM5	NULL		interacts with	NULL				CD36	NULL		immunodominant domain (aa 155-183)		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
40439	18	10673	6	NULL	NULL	0	NULL	statement 17	NULL		blocks	NULL				CD36	NULL	function of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
40441	19	10673	6	NULL	NULL	0	NULL	FA6-152	NULL		interacts with	NULL				CD36	NULL		immunodominant domain (aa 155-183)		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
40443	20	10673	6	NULL	NULL	0	NULL	statement 19	NULL		blocks	NULL				CD36	NULL	function of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
40444	21	10673	6	NULL	NULL	0	NULL	L103	NULL		interacts with	NULL				CD36	NULL		immunodominant domain (aa 155-183)		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
40445	22	10673	6	NULL	NULL	0	NULL	statement 21	NULL		blocks	NULL				CD36	NULL	function of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
40446	23	10673	6	NULL	NULL	0	NULL	5F1	NULL		interacts with	NULL				CD36	NULL		immunodominant domain (aa 155-183)		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
40447	24	10673	6	NULL	NULL	0	NULL	statement 23	NULL		blocks	NULL				CD36	NULL	function of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
40448	25	10673	6	NULL	NULL	0	NULL	Smphi	NULL		interacts with	NULL				CD36	NULL		immunodominant domain (aa 155-183)		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
40449	26	10673	6	NULL	NULL	0	NULL	statement 25	NULL		blocks	NULL				CD36	NULL	function of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
40450	27	10673	6	NULL	NULL	0	NULL	ESIVC7	NULL		interacts with	NULL				CD36	NULL		immunodominant domain (aa 155-183)		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
40451	28	10673	6	NULL	NULL	0	NULL	statement 27	NULL		blocks	NULL				CD36	NULL	function of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
40454	29	10673	6	NULL	NULL	0	NULL	10/5	NULL		interacts with	NULL				CD36	NULL		immunodominant domain (aa 155-183)		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
40456	30	10673	6	NULL	NULL	0	NULL	statement 29	NULL		blocks	NULL				CD36	NULL	function of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_52_34875_s_36	9857015	A large group of monoclonal antibodies raised in different laboratories against human CD36 ( e.g. 8A6, OKM5, FA6-152, L103, 5F1, Smphi, ESIVC7, and 10/5) have been shown to interact with an immunodominant domain spanning amino acids 155-183 ( 50,  51,  54) and to block numerous unrelated CD36 functions including TSP binding ( 52,  53), collagen binding ( 55), malaria cytoadhesion ( 56), uptake of apoptotic cells ( 44) and ROS ( 35), and Ox-LDL binding ( 25,  26).	bind
47440	1	10674	5	13	NULL	NULL	NULL	pericentrin B/kendrin	GP	large isoform	is homologous to					Spc110p	GP		calmodulin binding domain		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_8_3642_s_26	15146056	A large isoform (pericentrin B/kendrin; Flory and Davis, 2003 ) and another centrosome protein called AKAP450/GC-NAP share homology with the calmodulin binding domain of Spc110p (Flory  et al., 2000 ; Gillingham and Munro, 2000 ; Li  et al., 2001 ).	bind
47441	2	10674	5	13	NULL	NULL	NULL	AKAP450/GC-NAP	GP		is homologous to					Spc110p	GP		calmodulin binding domain		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_8_3642_s_26	15146056	A large isoform (pericentrin B/kendrin; Flory and Davis, 2003 ) and another centrosome protein called AKAP450/GC-NAP share homology with the calmodulin binding domain of Spc110p (Flory  et al., 2000 ; Gillingham and Munro, 2000 ; Li  et al., 2001 ).	bind
47442	3	10674	5	13	NULL	NULL	NULL	AKAP450/GC-NAP	GP		is a type of					centrosome protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_8_3642_s_26	15146056	A large isoform (pericentrin B/kendrin; Flory and Davis, 2003 ) and another centrosome protein called AKAP450/GC-NAP share homology with the calmodulin binding domain of Spc110p (Flory  et al., 2000 ; Gillingham and Munro, 2000 ; Li  et al., 2001 ).	bind
40051	1	10674	6	10	NULL	0	NULL	pericentrin B/kendrin	NULL	large isoform	is homologous to	NULL				Spc110p	NULL		calmodulin binding domain		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_8_3642_s_26	15146056	A large isoform (pericentrin B/kendrin; Flory and Davis, 2003 ) and another centrosome protein called AKAP450/GC-NAP share homology with the calmodulin binding domain of Spc110p (Flory  et al., 2000 ; Gillingham and Munro, 2000 ; Li  et al., 2001 ).	bind
40053	2	10674	6	NULL	NULL	0	NULL	AKAP450/GC-NAP	NULL		is a type of	NULL				centrosome protein	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_8_3642_s_26	15146056	A large isoform (pericentrin B/kendrin; Flory and Davis, 2003 ) and another centrosome protein called AKAP450/GC-NAP share homology with the calmodulin binding domain of Spc110p (Flory  et al., 2000 ; Gillingham and Munro, 2000 ; Li  et al., 2001 ).	bind
40056	3	10674	6	NULL	NULL	0	NULL	AKAP450/GC-NAP	NULL		is homologous to	NULL				Spc110p	NULL		calmodulin binding domain		NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_8_3642_s_26	15146056	A large isoform (pericentrin B/kendrin; Flory and Davis, 2003 ) and another centrosome protein called AKAP450/GC-NAP share homology with the calmodulin binding domain of Spc110p (Flory  et al., 2000 ; Gillingham and Munro, 2000 ; Li  et al., 2001 ).	bind
47445	1	10677	5	13	NULL	NULL	NULL	HCV peptide	GP		bind					HLA-A2	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_58_0_391_s_214	15487943	A large number of HCV epitopes have been identified either by predictive  algorithms for HCV peptide binding to common MHC molecules such as HLA-A2 ( 10, 16) or by mapping with virus-specific CD8+ T cell populations recovered from blood or  liver of infected individuals.	bind
47446	2	10677	5	13	NULL	NULL	NULL	HLA-A2	GP		is a type of					MHC molecule	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_58_0_391_s_214	15487943	A large number of HCV epitopes have been identified either by predictive  algorithms for HCV peptide binding to common MHC molecules such as HLA-A2 ( 10, 16) or by mapping with virus-specific CD8+ T cell populations recovered from blood or  liver of infected individuals.	bind
40411	1	10677	6	NULL	NULL	0	NULL	HCV peptide	NULL		bind	NULL				HLA-A2	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_58_0_391_s_214	15487943	A large number of HCV epitopes have been identified either by predictive  algorithms for HCV peptide binding to common MHC molecules such as HLA-A2 ( 10, 16) or by mapping with virus-specific CD8+ T cell populations recovered from blood or  liver of infected individuals.	bind
40412	2	10677	6	NULL	NULL	0	NULL	HLA-A2	NULL		is a type of	NULL				MHC molecules	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_58_0_391_s_214	15487943	A large number of HCV epitopes have been identified either by predictive  algorithms for HCV peptide binding to common MHC molecules such as HLA-A2 ( 10, 16) or by mapping with virus-specific CD8+ T cell populations recovered from blood or  liver of infected individuals.	bind
47447	1	10678	5	13	NULL	NULL	NULL	PcGs	GP		bind					neuronal differentiation genes	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_20_9_1123_s_157	16618801	A large number of neuronal differentiation genes are bound by PcGs (Table  1).	bind
40061	1	10678	6	10	NULL	0	NULL	PcGs	NULL		bind	NULL				 neuronal differentiation genes	NULL				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_20_9_1123_s_157	16618801	A large number of neuronal differentiation genes are bound by PcGs (Table  1).	bind
47448	1	10679	5	13	NULL	NULL	NULL	complexins	GP		bind					syntaxin	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_26_1_45_s_20	10798391	A large number of proteins have been identified which bind to SNARE proteins and have been implicated in regulating SNARE complex formation: complexins, Munc-13, Munc-18, syncollin, syntaphilin, and tomosyn bind to syntaxin; HRS-2 and snapin bind to SNAP-25; and VAP-33 binds to VAMP (   Skehel, 1995  ; Bean et al. 1997  ; Edwardson, 1997  ; Mochida et al., 2000).	bind
47449	2	10679	5	13	NULL	NULL	NULL	Munc-13	GP		bind					syntaxin	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_26_1_45_s_20	10798391	A large number of proteins have been identified which bind to SNARE proteins and have been implicated in regulating SNARE complex formation: complexins, Munc-13, Munc-18, syncollin, syntaphilin, and tomosyn bind to syntaxin; HRS-2 and snapin bind to SNAP-25; and VAP-33 binds to VAMP (   Skehel, 1995  ; Bean et al. 1997  ; Edwardson, 1997  ; Mochida et al., 2000).	bind
47450	3	10679	5	13	NULL	NULL	NULL	Munc-18	GP		bind					syntaxin	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_26_1_45_s_20	10798391	A large number of proteins have been identified which bind to SNARE proteins and have been implicated in regulating SNARE complex formation: complexins, Munc-13, Munc-18, syncollin, syntaphilin, and tomosyn bind to syntaxin; HRS-2 and snapin bind to SNAP-25; and VAP-33 binds to VAMP (   Skehel, 1995  ; Bean et al. 1997  ; Edwardson, 1997  ; Mochida et al., 2000).	bind
47451	4	10679	5	13	NULL	NULL	NULL	syncollin	GP		bind					syntaxin	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_26_1_45_s_20	10798391	A large number of proteins have been identified which bind to SNARE proteins and have been implicated in regulating SNARE complex formation: complexins, Munc-13, Munc-18, syncollin, syntaphilin, and tomosyn bind to syntaxin; HRS-2 and snapin bind to SNAP-25; and VAP-33 binds to VAMP (   Skehel, 1995  ; Bean et al. 1997  ; Edwardson, 1997  ; Mochida et al., 2000).	bind
47452	5	10679	5	13	NULL	NULL	NULL	syntaphilin	GP		bind					syntaxin	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_26_1_45_s_20	10798391	A large number of proteins have been identified which bind to SNARE proteins and have been implicated in regulating SNARE complex formation: complexins, Munc-13, Munc-18, syncollin, syntaphilin, and tomosyn bind to syntaxin; HRS-2 and snapin bind to SNAP-25; and VAP-33 binds to VAMP (   Skehel, 1995  ; Bean et al. 1997  ; Edwardson, 1997  ; Mochida et al., 2000).	bind
47453	6	10679	5	13	NULL	NULL	NULL	tomosyn	GP		bind					syntaxin	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_26_1_45_s_20	10798391	A large number of proteins have been identified which bind to SNARE proteins and have been implicated in regulating SNARE complex formation: complexins, Munc-13, Munc-18, syncollin, syntaphilin, and tomosyn bind to syntaxin; HRS-2 and snapin bind to SNAP-25; and VAP-33 binds to VAMP (   Skehel, 1995  ; Bean et al. 1997  ; Edwardson, 1997  ; Mochida et al., 2000).	bind
47454	7	10679	5	13	NULL	NULL	NULL	HRS-2	GP		bind					SNAP-25	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_26_1_45_s_20	10798391	A large number of proteins have been identified which bind to SNARE proteins and have been implicated in regulating SNARE complex formation: complexins, Munc-13, Munc-18, syncollin, syntaphilin, and tomosyn bind to syntaxin; HRS-2 and snapin bind to SNAP-25; and VAP-33 binds to VAMP (   Skehel, 1995  ; Bean et al. 1997  ; Edwardson, 1997  ; Mochida et al., 2000).	bind
47455	8	10679	5	13	NULL	NULL	NULL	snapin	GP		bind					SNAP-25	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_26_1_45_s_20	10798391	A large number of proteins have been identified which bind to SNARE proteins and have been implicated in regulating SNARE complex formation: complexins, Munc-13, Munc-18, syncollin, syntaphilin, and tomosyn bind to syntaxin; HRS-2 and snapin bind to SNAP-25; and VAP-33 binds to VAMP (   Skehel, 1995  ; Bean et al. 1997  ; Edwardson, 1997  ; Mochida et al., 2000).	bind
47456	9	10679	5	13	NULL	NULL	NULL	VAP-33	GP		bind					VAMP	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_26_1_45_s_20	10798391	A large number of proteins have been identified which bind to SNARE proteins and have been implicated in regulating SNARE complex formation: complexins, Munc-13, Munc-18, syncollin, syntaphilin, and tomosyn bind to syntaxin; HRS-2 and snapin bind to SNAP-25; and VAP-33 binds to VAMP (   Skehel, 1995  ; Bean et al. 1997  ; Edwardson, 1997  ; Mochida et al., 2000).	bind
40062	1	10679	6	NULL	NULL	0	NULL	complexins	NULL		bind	NULL				syntaxin	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_26_1_45_s_20	10798391	A large number of proteins have been identified which bind to SNARE proteins and have been implicated in regulating SNARE complex formation: complexins, Munc-13, Munc-18, syncollin, syntaphilin, and tomosyn bind to syntaxin; HRS-2 and snapin bind to SNAP-25; and VAP-33 binds to VAMP (   Skehel, 1995  ; Bean et al. 1997  ; Edwardson, 1997  ; Mochida et al., 2000).	bind
40063	2	10679	6	NULL	NULL	0	NULL	Munc-13	NULL		bind	NULL				syntaxin	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_26_1_45_s_20	10798391	A large number of proteins have been identified which bind to SNARE proteins and have been implicated in regulating SNARE complex formation: complexins, Munc-13, Munc-18, syncollin, syntaphilin, and tomosyn bind to syntaxin; HRS-2 and snapin bind to SNAP-25; and VAP-33 binds to VAMP (   Skehel, 1995  ; Bean et al. 1997  ; Edwardson, 1997  ; Mochida et al., 2000).	bind
40065	3	10679	6	NULL	NULL	0	NULL	Munc-18	NULL		bind	NULL				syntaxin	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_26_1_45_s_20	10798391	A large number of proteins have been identified which bind to SNARE proteins and have been implicated in regulating SNARE complex formation: complexins, Munc-13, Munc-18, syncollin, syntaphilin, and tomosyn bind to syntaxin; HRS-2 and snapin bind to SNAP-25; and VAP-33 binds to VAMP (   Skehel, 1995  ; Bean et al. 1997  ; Edwardson, 1997  ; Mochida et al., 2000).	bind
40067	4	10679	6	NULL	NULL	0	NULL	syncollin	NULL		bind	NULL				syntaxin	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_26_1_45_s_20	10798391	A large number of proteins have been identified which bind to SNARE proteins and have been implicated in regulating SNARE complex formation: complexins, Munc-13, Munc-18, syncollin, syntaphilin, and tomosyn bind to syntaxin; HRS-2 and snapin bind to SNAP-25; and VAP-33 binds to VAMP (   Skehel, 1995  ; Bean et al. 1997  ; Edwardson, 1997  ; Mochida et al., 2000).	bind
40069	5	10679	6	NULL	NULL	0	NULL	syntaphilin	NULL		bind	NULL				syntaxin	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_26_1_45_s_20	10798391	A large number of proteins have been identified which bind to SNARE proteins and have been implicated in regulating SNARE complex formation: complexins, Munc-13, Munc-18, syncollin, syntaphilin, and tomosyn bind to syntaxin; HRS-2 and snapin bind to SNAP-25; and VAP-33 binds to VAMP (   Skehel, 1995  ; Bean et al. 1997  ; Edwardson, 1997  ; Mochida et al., 2000).	bind
40070	6	10679	6	NULL	NULL	0	NULL	tomosyn	NULL		bind	NULL				syntaxin	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_26_1_45_s_20	10798391	A large number of proteins have been identified which bind to SNARE proteins and have been implicated in regulating SNARE complex formation: complexins, Munc-13, Munc-18, syncollin, syntaphilin, and tomosyn bind to syntaxin; HRS-2 and snapin bind to SNAP-25; and VAP-33 binds to VAMP (   Skehel, 1995  ; Bean et al. 1997  ; Edwardson, 1997  ; Mochida et al., 2000).	bind
40071	7	10679	6	NULL	NULL	0	NULL	HRS-2	NULL		bind	NULL				SNAP-25	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_26_1_45_s_20	10798391	A large number of proteins have been identified which bind to SNARE proteins and have been implicated in regulating SNARE complex formation: complexins, Munc-13, Munc-18, syncollin, syntaphilin, and tomosyn bind to syntaxin; HRS-2 and snapin bind to SNAP-25; and VAP-33 binds to VAMP (   Skehel, 1995  ; Bean et al. 1997  ; Edwardson, 1997  ; Mochida et al., 2000).	bind
40072	8	10679	6	NULL	NULL	0	NULL	snapin	NULL		bind	NULL				SNAP-25	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_26_1_45_s_20	10798391	A large number of proteins have been identified which bind to SNARE proteins and have been implicated in regulating SNARE complex formation: complexins, Munc-13, Munc-18, syncollin, syntaphilin, and tomosyn bind to syntaxin; HRS-2 and snapin bind to SNAP-25; and VAP-33 binds to VAMP (   Skehel, 1995  ; Bean et al. 1997  ; Edwardson, 1997  ; Mochida et al., 2000).	bind
40073	9	10679	6	NULL	NULL	0	NULL	VAP-33	NULL		bind	NULL				VAMP	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_26_1_45_s_20	10798391	A large number of proteins have been identified which bind to SNARE proteins and have been implicated in regulating SNARE complex formation: complexins, Munc-13, Munc-18, syncollin, syntaphilin, and tomosyn bind to syntaxin; HRS-2 and snapin bind to SNAP-25; and VAP-33 binds to VAMP (   Skehel, 1995  ; Bean et al. 1997  ; Edwardson, 1997  ; Mochida et al., 2000).	bind
47457	1	10680	5	13	NULL	NULL	NULL	vinca alkaloids	Chemical		bind					tubulin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_29_30731_s_20	15123603	A large number of structurally diverse compounds, including many unusual peptides and depsipeptides, interfere with the binding of vinca alkaloids to tubulin.	bind
47458	2	10680	5	13	NULL	NULL	NULL	depsipeptides	GP		interfere with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_29_30731_s_20	15123603	A large number of structurally diverse compounds, including many unusual peptides and depsipeptides, interfere with the binding of vinca alkaloids to tubulin.	bind
40076	1	10680	6	NULL	NULL	0	NULL	vinca alkaloids	NULL		bind	NULL				tubulin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_29_30731_s_20	15123603	A large number of structurally diverse compounds, including many unusual peptides and depsipeptides, interfere with the binding of vinca alkaloids to tubulin.	bind
40077	2	10680	6	NULL	NULL	0	NULL	depsipeptides	NULL		interferes with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_29_30731_s_20	15123603	A large number of structurally diverse compounds, including many unusual peptides and depsipeptides, interfere with the binding of vinca alkaloids to tubulin.	bind
47459	1	10681	5	13	NULL	NULL	NULL	Cds1	GP		preserves					genome	NucleicAcid	integrity of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_8_919_s_56	15805465	A large number of studies have established that Cds1 and Rad53 are required for survival of replication stress, and some have demonstrated physical links between these proteins and others involved in genome maintenance, but there have been few mechanistic insights into exactly how Cds1 and Rad53 function to preserve genome integrity.	bind
47460	2	10681	5	13	NULL	NULL	NULL	Rad53	GP		preserves					genome	NucleicAcid	integrity of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_8_919_s_56	15805465	A large number of studies have established that Cds1 and Rad53 are required for survival of replication stress, and some have demonstrated physical links between these proteins and others involved in genome maintenance, but there have been few mechanistic insights into exactly how Cds1 and Rad53 function to preserve genome integrity.	bind
47461	3	10681	5	13	NULL	NULL	NULL	Cds1	GP		is required for					replication stress	Process	survival of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_8_919_s_56	15805465	A large number of studies have established that Cds1 and Rad53 are required for survival of replication stress, and some have demonstrated physical links between these proteins and others involved in genome maintenance, but there have been few mechanistic insights into exactly how Cds1 and Rad53 function to preserve genome integrity.	bind
47462	4	10681	5	13	NULL	NULL	NULL	Rad53	GP		is required for					replication stress	Process	survival of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_8_919_s_56	15805465	A large number of studies have established that Cds1 and Rad53 are required for survival of replication stress, and some have demonstrated physical links between these proteins and others involved in genome maintenance, but there have been few mechanistic insights into exactly how Cds1 and Rad53 function to preserve genome integrity.	bind
40470	1	10681	6	NULL	NULL	0	NULL	Cds1	NULL		is required for	NULL				replication stress	NULL	survival of			NULL		0	NULL	NULL	NULL	gw70_genesdev_19_8_919_s_56	15805465	A large number of studies have established that Cds1 and Rad53 are required for survival of replication stress, and some have demonstrated physical links between these proteins and others involved in genome maintenance, but there have been few mechanistic insights into exactly how Cds1 and Rad53 function to preserve genome integrity.	bind
40475	2	10681	6	NULL	NULL	0	NULL	Rad53	NULL		are required for	NULL				replication stress	NULL	survival of			NULL		0	NULL	NULL	NULL	gw70_genesdev_19_8_919_s_56	15805465	A large number of studies have established that Cds1 and Rad53 are required for survival of replication stress, and some have demonstrated physical links between these proteins and others involved in genome maintenance, but there have been few mechanistic insights into exactly how Cds1 and Rad53 function to preserve genome integrity.	bind
40477	3	10681	6	10	NULL	0	NULL	Cds1			preserves					genome 		integrity of 			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_8_919_s_56	15805465	A large number of studies have established that Cds1 and Rad53 are required for survival of replication stress, and some have demonstrated physical links between these proteins and others involved in genome maintenance, but there have been few mechanistic insights into exactly how Cds1 and Rad53 function to preserve genome integrity.	bind
40478	4	10681	6	10	NULL	0	NULL	Rad53			preserves					genome 		integrity of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_8_919_s_56	15805465	A large number of studies have established that Cds1 and Rad53 are required for survival of replication stress, and some have demonstrated physical links between these proteins and others involved in genome maintenance, but there have been few mechanistic insights into exactly how Cds1 and Rad53 function to preserve genome integrity.	bind
47463	1	10682	5	13	NULL	NULL	NULL	cells	Cell	porin-treated	bind					annexin V	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_2_339_s_118	9889191	A large percentage of the porin-treated cells bound annexin V (Figure  2D).	bind
40078	1	10682	6	NULL	NULL	0	NULL	porin-treated cells	NULL		bind	NULL				annexin V	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_18_2_339_s_118	9889191	A large percentage of the porin-treated cells bound annexin V (Figure  2D).	bind
47464	1	10683	5	13	NULL	NULL	NULL	mPIP5KIbeta	GP		colocalize with					PI(4,5)P2 microdomains	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_17_17346_s_209	15741173	A large population of mPIP5KIbeta was colocalized with PI(4,5)P2 microdomains ( B) and syntaxin clusters ( C).	bind
47465	2	10683	5	13	NULL	NULL	NULL	mPIP5KIbeta	GP		colocalize with					syntaxin clusters	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_17_17346_s_209	15741173	A large population of mPIP5KIbeta was colocalized with PI(4,5)P2 microdomains ( B) and syntaxin clusters ( C).	bind
40080	1	10683	6	NULL	NULL	0	NULL	mPIP5KIbeta	NULL		colocalizes with	NULL				PI(4,5)P2 microdomains	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_17_17346_s_209	15741173	A large population of mPIP5KIbeta was colocalized with PI(4,5)P2 microdomains ( B) and syntaxin clusters ( C).	bind
40081	2	10683	6	NULL	NULL	0	NULL	mPIP5KIbeta	NULL		colocalizes with	NULL				syntaxin clusters	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_17_17346_s_209	15741173	A large population of mPIP5KIbeta was colocalized with PI(4,5)P2 microdomains ( B) and syntaxin clusters ( C).	bind
47466	1	10684	5	13	NULL	NULL	NULL	TSP-4 particles	GP		bind					collagen molecules	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_47_37110_s_202	10956668	A large proportion of all TSP-4 particles was bound to collagen molecules.	bind
40082	1	10684	6	NULL	NULL	0	NULL	TSP-4 particles	NULL		bind	NULL				collagen molecules	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_47_37110_s_202	10956668	A large proportion of all TSP-4 particles was bound to collagen molecules.	bind
47467	1	10685	5	13	NULL	NULL	NULL	B-Myb	GP		complexes with					p107	GP				NULL	cotransfected cells	NULL	NULL	NULL	NULL	abs-batch0517-0529_oncogene_21_52_12439743_s_5	12439743	A large proportion of B-Myb formed complexes with p107 in cotransfected  cells, however, B-Myb bound weakly to the related p130 protein and not  at all to pRb.	bind
47468	2	10685	5	13	NULL	NULL	NULL	B-Myb	GP		bind		weakly			p130 protein	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_oncogene_21_52_12439743_s_5	12439743	A large proportion of B-Myb formed complexes with p107 in cotransfected  cells, however, B-Myb bound weakly to the related p130 protein and not  at all to pRb.	bind
47469	3	10685	5	13	NULL	NULL	NULL	B-Myb	GP		does not bind					pRb	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_oncogene_21_52_12439743_s_5	12439743	A large proportion of B-Myb formed complexes with p107 in cotransfected  cells, however, B-Myb bound weakly to the related p130 protein and not  at all to pRb.	bind
40084	1	10685	6	NULL	NULL	0	NULL	B-Myb	NULL		forms complexes with	NULL				p107	NULL				NULL	cotransfected cells	0	NULL	NULL	NULL	abs-batch0517-0529_oncogene_21_52_12439743_s_5	12439743	A large proportion of B-Myb formed complexes with p107 in cotransfected  cells, however, B-Myb bound weakly to the related p130 protein and not  at all to pRb.	bind
40085	2	10685	6	NULL	NULL	0	NULL	B-Myb	NULL		bind	NULL	weakly			p130 protein	NULL				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_oncogene_21_52_12439743_s_5	12439743	A large proportion of B-Myb formed complexes with p107 in cotransfected  cells, however, B-Myb bound weakly to the related p130 protein and not  at all to pRb.	bind
40086	3	10685	6	NULL	NULL	0	NULL	B-Myb	NULL		does not bind	NULL				pRb	NULL				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_oncogene_21_52_12439743_s_5	12439743	A large proportion of B-Myb formed complexes with p107 in cotransfected  cells, however, B-Myb bound weakly to the related p130 protein and not  at all to pRb.	bind
47507	1	10686	5	13	NULL	NULL	NULL	PLTP	GP		bind					apoA-I	GP				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_39_1_152_s_149	9469594	A large proportion of the applied PLTP activity (66%) bound to the apoA-I column, and could be recovered (84%) by elution with 0.5% CHAPS in PBS.	bind
40099	1	10686	6	NULL	NULL	0	NULL	PLTP	NULL		bind	NULL				apoA-I	NULL				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_1_152_s_149	9469594	A large proportion of the applied PLTP activity (66%) bound to the apoA-I column, and could be recovered (84%) by elution with 0.5% CHAPS in PBS.	bind
47508	1	10687	5	13	NULL	NULL	NULL	GABAA receptor subtype	GP	thalamus	does not bind			MUS binding sites		benzodiazepines	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_118_4_1033_s_209	12732248	A large proportion of [3]MUS binding sites in the thalamus is thought to be a part of the GABAA receptor subtype that does not bind benzodiazepines ( Unnerstal et al., 1981).	bind
40100	1	10687	6	10	NULL	0	NULL	GABAA receptor subtype	NULL	thalamus	does not bind	NULL		MUS binding sites		benzodiazepines	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_118_4_1033_s_209	12732248	A large proportion of [3]MUS binding sites in the thalamus is thought to be a part of the GABAA receptor subtype that does not bind benzodiazepines ( Unnerstal et al., 1981).	bind
47501	1	10688	5	13	NULL	NULL	NULL	Ypt7	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_318_1_148_s_209	15110766	A large protein complex containing vps39 and vps41 functions  as a downstream effector of the active, GTP-bound form of Ypt7, a rab GTPase required  for the fusion of vesicular intermediates with a vacuole [ 51].	bind
47502	2	10688	5	13	NULL	NULL	NULL	vps39	GP		is in complex with					vps41	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_318_1_148_s_209	15110766	A large protein complex containing vps39 and vps41 functions  as a downstream effector of the active, GTP-bound form of Ypt7, a rab GTPase required  for the fusion of vesicular intermediates with a vacuole [ 51].	bind
47503	3	10688	5	13	NULL	NULL	NULL	statement 2	Process		function as					statement 1	Process	downstream effector of;;active			NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_318_1_148_s_209	15110766	A large protein complex containing vps39 and vps41 functions  as a downstream effector of the active, GTP-bound form of Ypt7, a rab GTPase required  for the fusion of vesicular intermediates with a vacuole [ 51].	bind
47504	4	10688	5	13	NULL	NULL	NULL	Ypt7	GP		is a type of					rab GTPase	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_318_1_148_s_209	15110766	A large protein complex containing vps39 and vps41 functions  as a downstream effector of the active, GTP-bound form of Ypt7, a rab GTPase required  for the fusion of vesicular intermediates with a vacuole [ 51].	bind
47505	5	10688	5	13	NULL	NULL	NULL	vesicular intermediates	CellComponent		fuse with					vacuole	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_318_1_148_s_209	15110766	A large protein complex containing vps39 and vps41 functions  as a downstream effector of the active, GTP-bound form of Ypt7, a rab GTPase required  for the fusion of vesicular intermediates with a vacuole [ 51].	bind
50252	6	10688	5	13	NULL	NULL	NULL	Ypt7	GP		is required for					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_318_1_148_s_209	15110766	A large protein complex containing vps39 and vps41 functions  as a downstream effector of the active, GTP-bound form of Ypt7, a rab GTPase required  for the fusion of vesicular intermediates with a vacuole [ 51].	bind
40413	1	10688	6	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				Ypt7	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_318_1_148_s_209	15110766	A large protein complex containing vps39 and vps41 functions  as a downstream effector of the active, GTP-bound form of Ypt7, a rab GTPase required  for the fusion of vesicular intermediates with a vacuole [ 51].	bind
40414	2	10688	6	NULL	NULL	0	NULL	Ypt7	NULL		is a type of	NULL				rab GTPase	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_318_1_148_s_209	15110766	A large protein complex containing vps39 and vps41 functions  as a downstream effector of the active, GTP-bound form of Ypt7, a rab GTPase required  for the fusion of vesicular intermediates with a vacuole [ 51].	bind
40415	3	10688	6	10	NULL	0	NULL	vesicular intermediates	NULL		fuse with	NULL				vacuole	NULL				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_318_1_148_s_209	15110766	A large protein complex containing vps39 and vps41 functions  as a downstream effector of the active, GTP-bound form of Ypt7, a rab GTPase required  for the fusion of vesicular intermediates with a vacuole [ 51].	bind
40416	4	10688	6	NULL	NULL	0	NULL	vps39	NULL		forms a complex with	NULL				vps41	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_318_1_148_s_209	15110766	A large protein complex containing vps39 and vps41 functions  as a downstream effector of the active, GTP-bound form of Ypt7, a rab GTPase required  for the fusion of vesicular intermediates with a vacuole [ 51].	bind
40417	5	10688	6	NULL	NULL	0	NULL	statement 4	NULL		acts as 	NULL				statement 1	NULL	downstream effector of;; active			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_318_1_148_s_209	15110766	A large protein complex containing vps39 and vps41 functions  as a downstream effector of the active, GTP-bound form of Ypt7, a rab GTPase required  for the fusion of vesicular intermediates with a vacuole [ 51].	bind
50253	6	10688	6	10	NULL	0	NULL	Ypt7	NULL		is required for	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_318_1_148_s_209	15110766	A large protein complex containing vps39 and vps41 functions  as a downstream effector of the active, GTP-bound form of Ypt7, a rab GTPase required  for the fusion of vesicular intermediates with a vacuole [ 51].	bind
47509	1	10689	5	13	NULL	NULL	NULL	EB	Chemical		bind					CHO-18.4 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_74_3_1795_s_75	16495553	A large reduction in EB binding to CHO-18.4 cells was not observed, suggesting that the specific lack of heparan sulfate on the surface of CHO cells had little effect on the ability of EB to attach to host cells.	bind
47510	2	10689	5	13	NULL	NULL	NULL	CHO cells	Cell	surface of	lacks					heparan sulfate	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_74_3_1795_s_75	16495553	A large reduction in EB binding to CHO-18.4 cells was not observed, suggesting that the specific lack of heparan sulfate on the surface of CHO cells had little effect on the ability of EB to attach to host cells.	bind
47511	3	10689	5	13	NULL	NULL	NULL	statement 2	Process		has little effect on					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_infectimmun_74_3_1795_s_75	16495553	A large reduction in EB binding to CHO-18.4 cells was not observed, suggesting that the specific lack of heparan sulfate on the surface of CHO cells had little effect on the ability of EB to attach to host cells.	bind
40101	1	10689	6	NULL	NULL	0	NULL	EB	NULL		bind	NULL				CHO-18.4 cells	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_74_3_1795_s_75	16495553	A large reduction in EB binding to CHO-18.4 cells was not observed, suggesting that the specific lack of heparan sulfate on the surface of CHO cells had little effect on the ability of EB to attach to host cells.	bind
50254	2	10689	6	10	NULL	0	NULL	CHO cells	NULL	surface of	lack	NULL				 heparan sulfate	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_74_3_1795_s_75	16495553	A large reduction in EB binding to CHO-18.4 cells was not observed, suggesting that the specific lack of heparan sulfate on the surface of CHO cells had little effect on the ability of EB to attach to host cells.	bind
50255	3	10689	6	10	NULL	0	NULL	statement 2	NULL		has little effect on	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_74_3_1795_s_75	16495553	A large reduction in EB binding to CHO-18.4 cells was not observed, suggesting that the specific lack of heparan sulfate on the surface of CHO cells had little effect on the ability of EB to attach to host cells.	bind
47512	1	10690	5	13	NULL	NULL	NULL	p300	GP		bind					HIF-alpha 	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_11_9899_s_154	14701857	A larger decrease in O2 concentration is needed for a significant decrease in the activity of FIH, which allows binding of p300 to HIF-alpha and thus leads to maximal transcriptional activity.	bind
47513	2	10690	5	13	NULL	NULL	NULL	O2	Chemical	decrease in;;concentration of	is needed for					FIH	GP	decrease in;;activity of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_11_9899_s_154	14701857	A larger decrease in O2 concentration is needed for a significant decrease in the activity of FIH, which allows binding of p300 to HIF-alpha and thus leads to maximal transcriptional activity.	bind
47514	3	10690	5	13	NULL	NULL	NULL	statement 2	Process		allows					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_11_9899_s_154	14701857	A larger decrease in O2 concentration is needed for a significant decrease in the activity of FIH, which allows binding of p300 to HIF-alpha and thus leads to maximal transcriptional activity.	bind
47515	4	10690	5	13	NULL	NULL	NULL	statement 3	Process		leads to					transcriptional activity	Process	maximal			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_11_9899_s_154	14701857	A larger decrease in O2 concentration is needed for a significant decrease in the activity of FIH, which allows binding of p300 to HIF-alpha and thus leads to maximal transcriptional activity.	bind
40172	1	10690	6	NULL	NULL	0	NULL	p300	NULL		bind	NULL				HIF-alpha	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_11_9899_s_154	14701857	A larger decrease in O2 concentration is needed for a significant decrease in the activity of FIH, which allows binding of p300 to HIF-alpha and thus leads to maximal transcriptional activity.	bind
40173	2	10690	6	NULL	NULL	0	NULL	O2 concentration	NULL	decrease in	is needed for	NULL				FIH	NULL	decrease in;; activity of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_11_9899_s_154	14701857	A larger decrease in O2 concentration is needed for a significant decrease in the activity of FIH, which allows binding of p300 to HIF-alpha and thus leads to maximal transcriptional activity.	bind
40174	3	10690	6	NULL	NULL	0	NULL	statement 2	NULL		allows	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_11_9899_s_154	14701857	A larger decrease in O2 concentration is needed for a significant decrease in the activity of FIH, which allows binding of p300 to HIF-alpha and thus leads to maximal transcriptional activity.	bind
40175	4	10690	6	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				transcriptional activity	NULL	maximal			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_11_9899_s_154	14701857	A larger decrease in O2 concentration is needed for a significant decrease in the activity of FIH, which allows binding of p300 to HIF-alpha and thus leads to maximal transcriptional activity.	bind
47574	1	10691	5	13	NULL	NULL	NULL	AML-1B	GP		is an isoform of					AML-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_17_10647_s_236	9553127	A larger isoform of AML-1, AML-1B has an N-terminal extension ( 26); the AML-1B antiserum is specific to AML-1 members, and it has only weak binding to human AML-2 and AML-3 ( 27), which are other members of the AML family ( 28).	bind
47576	2	10691	5	13	NULL	NULL	NULL	AML-1B antiserum	GP		is specific to					AML-1 members	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_17_10647_s_236	9553127	A larger isoform of AML-1, AML-1B has an N-terminal extension ( 26); the AML-1B antiserum is specific to AML-1 members, and it has only weak binding to human AML-2 and AML-3 ( 27), which are other members of the AML family ( 28).	bind
47577	3	10691	5	13	NULL	NULL	NULL	AML-1B antiserum	GP		bind		weakly			AML-2	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_17_10647_s_236	9553127	A larger isoform of AML-1, AML-1B has an N-terminal extension ( 26); the AML-1B antiserum is specific to AML-1 members, and it has only weak binding to human AML-2 and AML-3 ( 27), which are other members of the AML family ( 28).	bind
47578	4	10691	5	13	NULL	NULL	NULL	AML-1B antiserum	GP		bind		weakly			AML-3	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_17_10647_s_236	9553127	A larger isoform of AML-1, AML-1B has an N-terminal extension ( 26); the AML-1B antiserum is specific to AML-1 members, and it has only weak binding to human AML-2 and AML-3 ( 27), which are other members of the AML family ( 28).	bind
47579	5	10691	5	13	NULL	NULL	NULL	AML-2	GP		is a member of					AML family	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_17_10647_s_236	9553127	A larger isoform of AML-1, AML-1B has an N-terminal extension ( 26); the AML-1B antiserum is specific to AML-1 members, and it has only weak binding to human AML-2 and AML-3 ( 27), which are other members of the AML family ( 28).	bind
47580	6	10691	5	13	NULL	NULL	NULL	AML-3	GP		is a member of					AML family	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_17_10647_s_236	9553127	A larger isoform of AML-1, AML-1B has an N-terminal extension ( 26); the AML-1B antiserum is specific to AML-1 members, and it has only weak binding to human AML-2 and AML-3 ( 27), which are other members of the AML family ( 28).	bind
40481	1	10691	6	NULL	NULL	0	NULL	AML-1B antiserum	NULL		bind	NULL	weakly			AML-2	NULL	human			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_17_10647_s_236	9553127	A larger isoform of AML-1, AML-1B has an N-terminal extension ( 26); the AML-1B antiserum is specific to AML-1 members, and it has only weak binding to human AML-2 and AML-3 ( 27), which are other members of the AML family ( 28).	bind
40482	2	10691	6	NULL	NULL	0	NULL	AML-1B antiserum	NULL		bind	NULL	weakly			AML-3	NULL	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_17_10647_s_236	9553127	A larger isoform of AML-1, AML-1B has an N-terminal extension ( 26); the AML-1B antiserum is specific to AML-1 members, and it has only weak binding to human AML-2 and AML-3 ( 27), which are other members of the AML family ( 28).	bind
40485	3	10691	6	NULL	NULL	0	NULL	AML-1B	NULL		is an isoform of	NULL				AML-1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_17_10647_s_236	9553127	A larger isoform of AML-1, AML-1B has an N-terminal extension ( 26); the AML-1B antiserum is specific to AML-1 members, and it has only weak binding to human AML-2 and AML-3 ( 27), which are other members of the AML family ( 28).	bind
40486	4	10691	6	NULL	NULL	0	NULL	AML-2	NULL		is a member of	NULL				AML family	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_17_10647_s_236	9553127	A larger isoform of AML-1, AML-1B has an N-terminal extension ( 26); the AML-1B antiserum is specific to AML-1 members, and it has only weak binding to human AML-2 and AML-3 ( 27), which are other members of the AML family ( 28).	bind
40487	5	10691	6	NULL	NULL	0	NULL	AML-3	NULL		is a member of	NULL				AML family	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_17_10647_s_236	9553127	A larger isoform of AML-1, AML-1B has an N-terminal extension ( 26); the AML-1B antiserum is specific to AML-1 members, and it has only weak binding to human AML-2 and AML-3 ( 27), which are other members of the AML family ( 28).	bind
50256	6	10691	6	10	NULL	0	NULL	AML-1B antiserum	NULL		is specific to	NULL				AML-1 members	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_17_10647_s_236	9553127	A larger isoform of AML-1, AML-1B has an N-terminal extension ( 26); the AML-1B antiserum is specific to AML-1 members, and it has only weak binding to human AML-2 and AML-3 ( 27), which are other members of the AML family ( 28).	bind
47581	1	10694	5	13	NULL	NULL	NULL	UP1	GP		bind					TR2-6F	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_43_42300_s_96	12904298	A least squares superposition of Calphas from the structures of UP1 bound to TR2-6F and TR2 (d(TTAGGG)2) showed no significant differences (root mean square deviation = 0.23  Ang ).	bind
47582	2	10694	5	13	NULL	NULL	NULL	UP1	GP		bind					TR2	NucleicAcid			d(TTAGGG)2	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_43_42300_s_96	12904298	A least squares superposition of Calphas from the structures of UP1 bound to TR2-6F and TR2 (d(TTAGGG)2) showed no significant differences (root mean square deviation = 0.23  Ang ).	bind
40176	1	10694	6	NULL	NULL	0	NULL	UP1	NULL		bind	NULL				TR2-6F	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_43_42300_s_96	12904298	A least squares superposition of Calphas from the structures of UP1 bound to TR2-6F and TR2 (d(TTAGGG)2) showed no significant differences (root mean square deviation = 0.23  Ang ).	bind
40177	2	10694	6	NULL	NULL	0	NULL	UP1	NULL		bind	NULL				TR2	NULL			d(TTAGGG)2	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_43_42300_s_96	12904298	A least squares superposition of Calphas from the structures of UP1 bound to TR2-6F and TR2 (d(TTAGGG)2) showed no significant differences (root mean square deviation = 0.23  Ang ).	bind
47583	1	10697	5	13	NULL	NULL	NULL	RNP complex	GP		bind			L7Ae					C/D motif		NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_22_6524_s_216	14602911	A less rigid RNP complex with only one L7Ae bound to the C/D motif could account for the increased activity.	bind
40488	1	10697	6	NULL	NULL	0	NULL	RNP complex	NULL		bind	NULL		L7Ae			NULL		C/D motif		NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_31_22_6524_s_216	14602911	A less rigid RNP complex with only one L7Ae bound to the C/D motif could account for the increased activity.	bind
47585	1	10699	5	13	NULL	NULL	NULL	KCNQ1	GP		coordinates			leucine zipper motif in C-terminus		yotiao	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_annurevpharmacol_43_0_441_s_177	12540747	A leucine zipper motif in the C-terminus of KCNQ1 coordinates the binding of a  targeting protein yotiao ( 85,  86), which in turn binds to and recruits PKA and protein phosphatase 1 (PP1) to the  channel.	bind
47586	2	10699	5	13	NULL	NULL	NULL	yotiao	GP		bind					PKA	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevpharmacol_43_0_441_s_177	12540747	A leucine zipper motif in the C-terminus of KCNQ1 coordinates the binding of a  targeting protein yotiao ( 85,  86), which in turn binds to and recruits PKA and protein phosphatase 1 (PP1) to the  channel.	bind
47587	3	10699	5	13	NULL	NULL	NULL	yotiao	GP		bind					PP1	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevpharmacol_43_0_441_s_177	12540747	A leucine zipper motif in the C-terminus of KCNQ1 coordinates the binding of a  targeting protein yotiao ( 85,  86), which in turn binds to and recruits PKA and protein phosphatase 1 (PP1) to the  channel.	bind
47588	4	10699	5	13	NULL	NULL	NULL	PP1	GP		is					protein phosphatase 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevpharmacol_43_0_441_s_177	12540747	A leucine zipper motif in the C-terminus of KCNQ1 coordinates the binding of a  targeting protein yotiao ( 85,  86), which in turn binds to and recruits PKA and protein phosphatase 1 (PP1) to the  channel.	bind
47589	5	10699	5	13	NULL	NULL	NULL	yotiao	GP		recruits					PKA	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevpharmacol_43_0_441_s_177	12540747	A leucine zipper motif in the C-terminus of KCNQ1 coordinates the binding of a  targeting protein yotiao ( 85,  86), which in turn binds to and recruits PKA and protein phosphatase 1 (PP1) to the  channel.	bind
47590	6	10699	5	13	NULL	NULL	NULL	yotiao	GP		recruits					PP1	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevpharmacol_43_0_441_s_177	12540747	A leucine zipper motif in the C-terminus of KCNQ1 coordinates the binding of a  targeting protein yotiao ( 85,  86), which in turn binds to and recruits PKA and protein phosphatase 1 (PP1) to the  channel.	bind
47591	7	10699	5	13	NULL	NULL	NULL	PKA	GP		is recruited to					channel	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevpharmacol_43_0_441_s_177	12540747	A leucine zipper motif in the C-terminus of KCNQ1 coordinates the binding of a  targeting protein yotiao ( 85,  86), which in turn binds to and recruits PKA and protein phosphatase 1 (PP1) to the  channel.	bind
47592	8	10699	5	13	NULL	NULL	NULL	PP1	GP		is recruited to					channel	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevpharmacol_43_0_441_s_177	12540747	A leucine zipper motif in the C-terminus of KCNQ1 coordinates the binding of a  targeting protein yotiao ( 85,  86), which in turn binds to and recruits PKA and protein phosphatase 1 (PP1) to the  channel.	bind
47593	9	10699	5	13	NULL	NULL	NULL	yotiao	GP		is a type of					targeting protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevpharmacol_43_0_441_s_177	12540747	A leucine zipper motif in the C-terminus of KCNQ1 coordinates the binding of a  targeting protein yotiao ( 85,  86), which in turn binds to and recruits PKA and protein phosphatase 1 (PP1) to the  channel.	bind
40489	1	10699	6	NULL	NULL	0	NULL	yotiao	NULL		bind	NULL				PKA	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevpharmacol_43_0_441_s_177	12540747	A leucine zipper motif in the C-terminus of KCNQ1 coordinates the binding of a  targeting protein yotiao ( 85,  86), which in turn binds to and recruits PKA and protein phosphatase 1 (PP1) to the  channel.	bind
40490	2	10699	6	NULL	NULL	0	NULL	yotiao	NULL		bind	NULL				PP1	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevpharmacol_43_0_441_s_177	12540747	A leucine zipper motif in the C-terminus of KCNQ1 coordinates the binding of a  targeting protein yotiao ( 85,  86), which in turn binds to and recruits PKA and protein phosphatase 1 (PP1) to the  channel.	bind
40491	3	10699	6	NULL	NULL	0	NULL	PP1	NULL		is	NULL				protein phosphatase 1	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevpharmacol_43_0_441_s_177	12540747	A leucine zipper motif in the C-terminus of KCNQ1 coordinates the binding of a  targeting protein yotiao ( 85,  86), which in turn binds to and recruits PKA and protein phosphatase 1 (PP1) to the  channel.	bind
40492	4	10699	6	NULL	NULL	0	NULL	yotiao	NULL		recruits	NULL				PKA	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevpharmacol_43_0_441_s_177	12540747	A leucine zipper motif in the C-terminus of KCNQ1 coordinates the binding of a  targeting protein yotiao ( 85,  86), which in turn binds to and recruits PKA and protein phosphatase 1 (PP1) to the  channel.	bind
40493	5	10699	6	NULL	NULL	0	NULL	PKA	NULL		is recruited to	NULL				channel	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevpharmacol_43_0_441_s_177	12540747	A leucine zipper motif in the C-terminus of KCNQ1 coordinates the binding of a  targeting protein yotiao ( 85,  86), which in turn binds to and recruits PKA and protein phosphatase 1 (PP1) to the  channel.	bind
40494	6	10699	6	NULL	NULL	0	NULL	PP1	NULL		is recruited to	NULL				channel	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevpharmacol_43_0_441_s_177	12540747	A leucine zipper motif in the C-terminus of KCNQ1 coordinates the binding of a  targeting protein yotiao ( 85,  86), which in turn binds to and recruits PKA and protein phosphatase 1 (PP1) to the  channel.	bind
40495	7	10699	6	NULL	NULL	0	NULL	yotiao	NULL		recruits	NULL				PP1	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevpharmacol_43_0_441_s_177	12540747	A leucine zipper motif in the C-terminus of KCNQ1 coordinates the binding of a  targeting protein yotiao ( 85,  86), which in turn binds to and recruits PKA and protein phosphatase 1 (PP1) to the  channel.	bind
40496	8	10699	6	NULL	NULL	0	NULL	yotiao	NULL		is a type of	NULL				targeting protein	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevpharmacol_43_0_441_s_177	12540747	A leucine zipper motif in the C-terminus of KCNQ1 coordinates the binding of a  targeting protein yotiao ( 85,  86), which in turn binds to and recruits PKA and protein phosphatase 1 (PP1) to the  channel.	bind
40497	9	10699	6	NULL	NULL	0	NULL	KCNQ1	NULL		coordinates	NULL		leucine zipper motif in C-terminus		yotiao	NULL	binding of			NULL		0	NULL	NULL	NULL	gw70_annurevpharmacol_43_0_441_s_177	12540747	A leucine zipper motif in the C-terminus of KCNQ1 coordinates the binding of a  targeting protein yotiao ( 85,  86), which in turn binds to and recruits PKA and protein phosphatase 1 (PP1) to the  channel.	bind
47594	1	10700	5	13	NULL	NULL	NULL	PAK	GP		is a type of					p21 GTPase-activated kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_34_26436_s_16	10840040	A leucine-rich motif that is repeated five times within the N terminus of paxillin binds a protein complex containing the p21 GTPase-activated kinase PAK, the adapter protein Nck, the guanine nucleotide exchange factor PIX, and the new multidomain ARF-GAP protein p95PKL (paxillin kinase linker) ( 11).	bind
47595	2	10700	5	13	NULL	NULL	NULL	Nck	GP		is a type of					adapter protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_34_26436_s_16	10840040	A leucine-rich motif that is repeated five times within the N terminus of paxillin binds a protein complex containing the p21 GTPase-activated kinase PAK, the adapter protein Nck, the guanine nucleotide exchange factor PIX, and the new multidomain ARF-GAP protein p95PKL (paxillin kinase linker) ( 11).	bind
47596	3	10700	5	13	NULL	NULL	NULL	PIX	GP		is a type of					guanine nucleotide exchange factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_34_26436_s_16	10840040	A leucine-rich motif that is repeated five times within the N terminus of paxillin binds a protein complex containing the p21 GTPase-activated kinase PAK, the adapter protein Nck, the guanine nucleotide exchange factor PIX, and the new multidomain ARF-GAP protein p95PKL (paxillin kinase linker) ( 11).	bind
47597	4	10700	5	13	NULL	NULL	NULL	p95PKL	GP		is					paxillin kinase linker	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_34_26436_s_16	10840040	A leucine-rich motif that is repeated five times within the N terminus of paxillin binds a protein complex containing the p21 GTPase-activated kinase PAK, the adapter protein Nck, the guanine nucleotide exchange factor PIX, and the new multidomain ARF-GAP protein p95PKL (paxillin kinase linker) ( 11).	bind
47598	5	10700	5	13	NULL	NULL	NULL	p95PKL	GP		is a type of					multidomain ARF-GAP protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_34_26436_s_16	10840040	A leucine-rich motif that is repeated five times within the N terminus of paxillin binds a protein complex containing the p21 GTPase-activated kinase PAK, the adapter protein Nck, the guanine nucleotide exchange factor PIX, and the new multidomain ARF-GAP protein p95PKL (paxillin kinase linker) ( 11).	bind
47599	6	10700	5	13	NULL	NULL	NULL	PAK	GP		is in complex with					Nck	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_34_26436_s_16	10840040	A leucine-rich motif that is repeated five times within the N terminus of paxillin binds a protein complex containing the p21 GTPase-activated kinase PAK, the adapter protein Nck, the guanine nucleotide exchange factor PIX, and the new multidomain ARF-GAP protein p95PKL (paxillin kinase linker) ( 11).	bind
47600	7	10700	5	13	NULL	NULL	NULL	statement 6	GP		is in complex with					PIX	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_34_26436_s_16	10840040	A leucine-rich motif that is repeated five times within the N terminus of paxillin binds a protein complex containing the p21 GTPase-activated kinase PAK, the adapter protein Nck, the guanine nucleotide exchange factor PIX, and the new multidomain ARF-GAP protein p95PKL (paxillin kinase linker) ( 11).	bind
47601	8	10700	5	13	NULL	NULL	NULL	statement 7	GP		is in complex with					p95PKL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_34_26436_s_16	10840040	A leucine-rich motif that is repeated five times within the N terminus of paxillin binds a protein complex containing the p21 GTPase-activated kinase PAK, the adapter protein Nck, the guanine nucleotide exchange factor PIX, and the new multidomain ARF-GAP protein p95PKL (paxillin kinase linker) ( 11).	bind
47602	9	10700	5	13	NULL	NULL	NULL	paxillin	GP		bind			leucine-rich motif within the N terminus		statement 8	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_34_26436_s_16	10840040	A leucine-rich motif that is repeated five times within the N terminus of paxillin binds a protein complex containing the p21 GTPase-activated kinase PAK, the adapter protein Nck, the guanine nucleotide exchange factor PIX, and the new multidomain ARF-GAP protein p95PKL (paxillin kinase linker) ( 11).	bind
40498	1	10700	6	NULL	NULL	0	NULL	PAK	NULL		is a type of	NULL				p21 GTPase-activated kinase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_34_26436_s_16	10840040	A leucine-rich motif that is repeated five times within the N terminus of paxillin binds a protein complex containing the p21 GTPase-activated kinase PAK, the adapter protein Nck, the guanine nucleotide exchange factor PIX, and the new multidomain ARF-GAP protein p95PKL (paxillin kinase linker) ( 11).	bind
40499	2	10700	6	NULL	NULL	0	NULL	Nck	NULL		is a type of	NULL				adapter protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_34_26436_s_16	10840040	A leucine-rich motif that is repeated five times within the N terminus of paxillin binds a protein complex containing the p21 GTPase-activated kinase PAK, the adapter protein Nck, the guanine nucleotide exchange factor PIX, and the new multidomain ARF-GAP protein p95PKL (paxillin kinase linker) ( 11).	bind
40500	3	10700	6	NULL	NULL	0	NULL	PIX	NULL		is a type of	NULL				guanine nucleotide exchange factor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_34_26436_s_16	10840040	A leucine-rich motif that is repeated five times within the N terminus of paxillin binds a protein complex containing the p21 GTPase-activated kinase PAK, the adapter protein Nck, the guanine nucleotide exchange factor PIX, and the new multidomain ARF-GAP protein p95PKL (paxillin kinase linker) ( 11).	bind
40501	4	10700	6	NULL	NULL	0	NULL	p95PKL	NULL		is a type of	NULL				multidomain ARF-GAP protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_34_26436_s_16	10840040	A leucine-rich motif that is repeated five times within the N terminus of paxillin binds a protein complex containing the p21 GTPase-activated kinase PAK, the adapter protein Nck, the guanine nucleotide exchange factor PIX, and the new multidomain ARF-GAP protein p95PKL (paxillin kinase linker) ( 11).	bind
40502	5	10700	6	NULL	NULL	0	NULL	PKL	NULL		is	NULL				paxillin kinase linker	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_34_26436_s_16	10840040	A leucine-rich motif that is repeated five times within the N terminus of paxillin binds a protein complex containing the p21 GTPase-activated kinase PAK, the adapter protein Nck, the guanine nucleotide exchange factor PIX, and the new multidomain ARF-GAP protein p95PKL (paxillin kinase linker) ( 11).	bind
40503	6	10700	6	NULL	NULL	0	NULL	PAK	NULL		forms a complex with	NULL				Nck	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_34_26436_s_16	10840040	A leucine-rich motif that is repeated five times within the N terminus of paxillin binds a protein complex containing the p21 GTPase-activated kinase PAK, the adapter protein Nck, the guanine nucleotide exchange factor PIX, and the new multidomain ARF-GAP protein p95PKL (paxillin kinase linker) ( 11).	bind
40504	7	10700	6	NULL	NULL	0	NULL	statement 6	NULL		forms a complex with	NULL				PIX	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_34_26436_s_16	10840040	A leucine-rich motif that is repeated five times within the N terminus of paxillin binds a protein complex containing the p21 GTPase-activated kinase PAK, the adapter protein Nck, the guanine nucleotide exchange factor PIX, and the new multidomain ARF-GAP protein p95PKL (paxillin kinase linker) ( 11).	bind
40505	8	10700	6	NULL	NULL	0	NULL	statement 7	NULL		forms a complex with	NULL				p95PKL	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_34_26436_s_16	10840040	A leucine-rich motif that is repeated five times within the N terminus of paxillin binds a protein complex containing the p21 GTPase-activated kinase PAK, the adapter protein Nck, the guanine nucleotide exchange factor PIX, and the new multidomain ARF-GAP protein p95PKL (paxillin kinase linker) ( 11).	bind
40506	9	10700	6	NULL	NULL	0	NULL	paxillin	NULL		bind	NULL		leucine-rich motif within N terminus		statement 8	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_34_26436_s_16	10840040	A leucine-rich motif that is repeated five times within the N terminus of paxillin binds a protein complex containing the p21 GTPase-activated kinase PAK, the adapter protein Nck, the guanine nucleotide exchange factor PIX, and the new multidomain ARF-GAP protein p95PKL (paxillin kinase linker) ( 11).	bind
47603	1	10701	5	13	NULL	NULL	NULL	NXF3	GP		is essential for			leucine-rich motif (296 to 302)		Crm1	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_2_397_s_202	11545741	A leucine-rich motif that mapped to around residues 296 to 302 in NXF3   (Figure 1A) was in fact found to be essential for both Crm1 binding and nuclear export mediated by the NXF3 protein    (Figures 2A and 4A).	bind
47604	2	10701	5	13	NULL	NULL	NULL	NXF3 protein	GP		mediate					nuclear export	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_2_397_s_202	11545741	A leucine-rich motif that mapped to around residues 296 to 302 in NXF3   (Figure 1A) was in fact found to be essential for both Crm1 binding and nuclear export mediated by the NXF3 protein    (Figures 2A and 4A).	bind
47605	3	10701	5	13	NULL	NULL	NULL	NXF3	GP		is essential for			leucine-rich motif (296 to 302)		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_2_397_s_202	11545741	A leucine-rich motif that mapped to around residues 296 to 302 in NXF3   (Figure 1A) was in fact found to be essential for both Crm1 binding and nuclear export mediated by the NXF3 protein    (Figures 2A and 4A).	bind
46902	1	10701	6	NULL	NULL	0	NULL	NXF3	NULL		is essential for	NULL		leucine rich motif;; 296-302		Crm1	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_2_397_s_202	11545741	A leucine-rich motif that mapped to around residues 296 to 302 in NXF3   (Figure 1A) was in fact found to be essential for both Crm1 binding and nuclear export mediated by the NXF3 protein    (Figures 2A and 4A).	bind
46903	2	10701	6	NULL	NULL	0	NULL	NXF3 protein	NULL		mediates	NULL				nuclear export	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_8_2_397_s_202	11545741	A leucine-rich motif that mapped to around residues 296 to 302 in NXF3   (Figure 1A) was in fact found to be essential for both Crm1 binding and nuclear export mediated by the NXF3 protein    (Figures 2A and 4A).	bind
46905	3	10701	6	NULL	NULL	0	NULL	NXF3	NULL		is essential for	NULL		leucine rich motif;; 296-302		statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_8_2_397_s_202	11545741	A leucine-rich motif that mapped to around residues 296 to 302 in NXF3   (Figure 1A) was in fact found to be essential for both Crm1 binding and nuclear export mediated by the NXF3 protein    (Figures 2A and 4A).	bind
47606	1	10703	5	13	NULL	NULL	NULL	long chain fatty acyl-CoA thioesters	Chemical		bind					HNF-4	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34105_s_227	9852068	A ligand for COUP-TF has not yet been identified, but it has recently been reported that long chain fatty acyl-CoA thioesters bind HNF-4 and enhance its ability to dimerize and bind DNA ( 44).	bind
47607	2	10703	5	13	NULL	NULL	NULL	HNF-4	GP		undergoes					dimerization	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34105_s_227	9852068	A ligand for COUP-TF has not yet been identified, but it has recently been reported that long chain fatty acyl-CoA thioesters bind HNF-4 and enhance its ability to dimerize and bind DNA ( 44).	bind
47608	3	10703	5	13	NULL	NULL	NULL	HNF-4	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34105_s_227	9852068	A ligand for COUP-TF has not yet been identified, but it has recently been reported that long chain fatty acyl-CoA thioesters bind HNF-4 and enhance its ability to dimerize and bind DNA ( 44).	bind
47609	4	10703	5	13	NULL	NULL	NULL	statement 1	Process		enhance					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34105_s_227	9852068	A ligand for COUP-TF has not yet been identified, but it has recently been reported that long chain fatty acyl-CoA thioesters bind HNF-4 and enhance its ability to dimerize and bind DNA ( 44).	bind
47610	5	10703	5	13	NULL	NULL	NULL	statement 1	Process		enhance					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34105_s_227	9852068	A ligand for COUP-TF has not yet been identified, but it has recently been reported that long chain fatty acyl-CoA thioesters bind HNF-4 and enhance its ability to dimerize and bind DNA ( 44).	bind
46906	1	10703	6	NULL	NULL	0	NULL	long chain fatty acyl-CoA thioesters	NULL		bind	NULL				HNF4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_51_34105_s_227	9852068	A ligand for COUP-TF has not yet been identified, but it has recently been reported that long chain fatty acyl-CoA thioesters bind HNF-4 and enhance its ability to dimerize and bind DNA ( 44).	bind
46907	2	10703	6	NULL	NULL	0	NULL	HNF4	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_51_34105_s_227	9852068	A ligand for COUP-TF has not yet been identified, but it has recently been reported that long chain fatty acyl-CoA thioesters bind HNF-4 and enhance its ability to dimerize and bind DNA ( 44).	bind
46908	3	10703	6	10	NULL	0	NULL	HNF4	NULL		undergoes	NULL				dimerization	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34105_s_227	9852068	A ligand for COUP-TF has not yet been identified, but it has recently been reported that long chain fatty acyl-CoA thioesters bind HNF-4 and enhance its ability to dimerize and bind DNA ( 44).	bind
46909	4	10703	6	NULL	NULL	0	NULL	statement 1	NULL		enhances	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_51_34105_s_227	9852068	A ligand for COUP-TF has not yet been identified, but it has recently been reported that long chain fatty acyl-CoA thioesters bind HNF-4 and enhance its ability to dimerize and bind DNA ( 44).	bind
46910	5	10703	6	NULL	NULL	0	NULL	statement 1	NULL		enhances	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_51_34105_s_227	9852068	A ligand for COUP-TF has not yet been identified, but it has recently been reported that long chain fatty acyl-CoA thioesters bind HNF-4 and enhance its ability to dimerize and bind DNA ( 44).	bind
47611	1	10705	5	13	NULL	NULL	NULL	Rho1p	GP	yeast	bind		directly			Fks1p	GP	Candida homolog of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_53_38119_s_158	10608882	A ligand overlay assay with  Candida albicans Rho1p has shown that yeast Rho1p can directly bind to the  Candida homolog of Fks1p ( 39).	bind
46911	1	10705	6	10	NULL	0	NULL	Rho1p	NULL	yeast	bind	NULL	directly			Fks1p	NULL	Candida homolog			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_53_38119_s_158	10608882	A ligand overlay assay with  Candida albicans Rho1p has shown that yeast Rho1p can directly bind to the  Candida homolog of Fks1p ( 39).	bind
47612	1	10707	5	13	NULL	NULL	NULL	PILR-L ligand	GP		bind					PILR	GP	mouse			NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_23_0_225_s_497	15771571	A ligand, designated PILR-L, that binds both mouse PILR  and PILR  has been identified;  it is a small transmembrane-anchored cell surface protein with homology to the CD99  gene family ( 344).	bind
47613	2	10707	5	13	NULL	NULL	NULL	PILR-L ligand	GP		bind					PILR	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_23_0_225_s_497	15771571	A ligand, designated PILR-L, that binds both mouse PILR  and PILR  has been identified;  it is a small transmembrane-anchored cell surface protein with homology to the CD99  gene family ( 344).	bind
47614	3	10707	5	13	NULL	NULL	NULL	PILR-L ligand	GP		is a type of					small transmembrane-anchored cell surface protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_23_0_225_s_497	15771571	A ligand, designated PILR-L, that binds both mouse PILR  and PILR  has been identified;  it is a small transmembrane-anchored cell surface protein with homology to the CD99  gene family ( 344).	bind
47615	4	10707	5	13	NULL	NULL	NULL	PILR-L ligand	GP		has homology to					CD99 gene family	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_23_0_225_s_497	15771571	A ligand, designated PILR-L, that binds both mouse PILR  and PILR  has been identified;  it is a small transmembrane-anchored cell surface protein with homology to the CD99  gene family ( 344).	bind
46912	1	10707	6	NULL	NULL	0	NULL	PILR-L	NULL		bind	NULL				PILR	NULL	mouse			NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_23_0_225_s_497	15771571	A ligand, designated PILR-L, that binds both mouse PILR  and PILR  has been identified;  it is a small transmembrane-anchored cell surface protein with homology to the CD99  gene family ( 344).	bind
46913	2	10707	6	NULL	NULL	0	NULL	PILR-L	NULL		bind	NULL				PILR	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_23_0_225_s_497	15771571	A ligand, designated PILR-L, that binds both mouse PILR  and PILR  has been identified;  it is a small transmembrane-anchored cell surface protein with homology to the CD99  gene family ( 344).	bind
46914	3	10707	6	NULL	NULL	0	NULL	PILR-L	NULL		is a type of 	NULL				small transmembrane-anchored cell surface protein	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_23_0_225_s_497	15771571	A ligand, designated PILR-L, that binds both mouse PILR  and PILR  has been identified;  it is a small transmembrane-anchored cell surface protein with homology to the CD99  gene family ( 344).	bind
46915	4	10707	6	NULL	NULL	0	NULL	PILR-L	NULL		has homology to	NULL				CD99 gene family	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_23_0_225_s_497	15771571	A ligand, designated PILR-L, that binds both mouse PILR  and PILR  has been identified;  it is a small transmembrane-anchored cell surface protein with homology to the CD99  gene family ( 344).	bind
47616	1	10709	5	13	NULL	NULL	NULL	Blimp-1	GP		is a member of					Groucho family of co-repressors	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_2_263_s_181	10637230	A likely candidate is Blimp-1, a member of the Groucho family of co-repressors that binds to the PRF site of the c- myc promoter and mediates repression (Lin  et al., 1997  ; Ren  et al., 1999)  .	bind
47617	2	10709	5	13	NULL	NULL	NULL	Blimp-1	GP		bind					c- myc	NucleicAcid			PRF site of promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_19_2_263_s_181	10637230	A likely candidate is Blimp-1, a member of the Groucho family of co-repressors that binds to the PRF site of the c- myc promoter and mediates repression (Lin  et al., 1997  ; Ren  et al., 1999)  .	bind
47618	3	10709	5	13	NULL	NULL	NULL	statement 2	Process		mediates					c-myc	GP	repression of 			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_2_263_s_181	10637230	A likely candidate is Blimp-1, a member of the Groucho family of co-repressors that binds to the PRF site of the c- myc promoter and mediates repression (Lin  et al., 1997  ; Ren  et al., 1999)  .	bind
46916	1	10709	6	NULL	NULL	0	NULL	Blimp-1	NULL		is a member of	NULL				Groucho family of co-repressors	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_19_2_263_s_181	10637230	A likely candidate is Blimp-1, a member of the Groucho family of co-repressors that binds to the PRF site of the c- myc promoter and mediates repression (Lin  et al., 1997  ; Ren  et al., 1999)  .	bind
46917	2	10709	6	NULL	NULL	0	NULL	Blimp-1	NULL		bind	NULL				c- myc	NULL			PRF site of promoter	NULL		0	NULL	NULL	NULL	gw60_embo_19_2_263_s_181	10637230	A likely candidate is Blimp-1, a member of the Groucho family of co-repressors that binds to the PRF site of the c- myc promoter and mediates repression (Lin  et al., 1997  ; Ren  et al., 1999)  .	bind
46918	3	10709	6	NULL	NULL	0	NULL	Blimp-1	NULL		mediates	NULL				c- myc	NULL	repression of		promoter	NULL		0	NULL	NULL	NULL	gw60_embo_19_2_263_s_181	10637230	A likely candidate is Blimp-1, a member of the Groucho family of co-repressors that binds to the PRF site of the c- myc promoter and mediates repression (Lin  et al., 1997  ; Ren  et al., 1999)  .	bind
47619	1	10710	5	13	NULL	NULL	NULL	Bax alpha	GP		bind					Bcl-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_10587_s_251	15590655	A likely explanation for the lack of activity detected with the latter mutant could be that mutation of Lys-64 enhanced the binding of Bax alpha to Bcl-2 (Fig. S4), and Asp-33 is central for the activation of Bax by proteases during apoptosis ( ,  ).	bind
47620	2	10710	5	13	NULL	NULL	NULL			mutation of	enhance			Lys-64		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_10587_s_251	15590655	A likely explanation for the lack of activity detected with the latter mutant could be that mutation of Lys-64 enhanced the binding of Bax alpha to Bcl-2 (Fig. S4), and Asp-33 is central for the activation of Bax by proteases during apoptosis ( ,  ).	bind
47621	3	10710	5	13	NULL	NULL	NULL	Bax	GP		is activated by					proteases	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_10587_s_251	15590655	A likely explanation for the lack of activity detected with the latter mutant could be that mutation of Lys-64 enhanced the binding of Bax alpha to Bcl-2 (Fig. S4), and Asp-33 is central for the activation of Bax by proteases during apoptosis ( ,  ).	bind
47622	4	10710	5	13	NULL	NULL	NULL				is essential for			Asp-33		statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_10587_s_251	15590655	A likely explanation for the lack of activity detected with the latter mutant could be that mutation of Lys-64 enhanced the binding of Bax alpha to Bcl-2 (Fig. S4), and Asp-33 is central for the activation of Bax by proteases during apoptosis ( ,  ).	bind
47623	5	10710	5	13	NULL	NULL	NULL	statement 4	Process		occurs during					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_10587_s_251	15590655	A likely explanation for the lack of activity detected with the latter mutant could be that mutation of Lys-64 enhanced the binding of Bax alpha to Bcl-2 (Fig. S4), and Asp-33 is central for the activation of Bax by proteases during apoptosis ( ,  ).	bind
46919	1	10710	6	NULL	NULL	0	NULL	Bax alpha	NULL		bind	NULL				Bcl-2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_11_10587_s_251	15590655	A likely explanation for the lack of activity detected with the latter mutant could be that mutation of Lys-64 enhanced the binding of Bax alpha to Bcl-2 (Fig. S4), and Asp-33 is central for the activation of Bax by proteases during apoptosis ( ,  ).	bind
46920	2	10710	6	NULL	NULL	0	NULL		NULL	mutation of	enhances	NULL		Lys-64		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_11_10587_s_251	15590655	A likely explanation for the lack of activity detected with the latter mutant could be that mutation of Lys-64 enhanced the binding of Bax alpha to Bcl-2 (Fig. S4), and Asp-33 is central for the activation of Bax by proteases during apoptosis ( ,  ).	bind
46921	4	10710	6	10	NULL	0	NULL		NULL		is essential for	NULL		Asp-33		statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_10587_s_251	15590655	A likely explanation for the lack of activity detected with the latter mutant could be that mutation of Lys-64 enhanced the binding of Bax alpha to Bcl-2 (Fig. S4), and Asp-33 is central for the activation of Bax by proteases during apoptosis ( ,  ).	bind
50302	3	10710	6	10	NULL	0	NULL	Bax	NULL		is activated by	NULL				proteases	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_11_10587_s_251	15590655	A likely explanation for the lack of activity detected with the latter mutant could be that mutation of Lys-64 enhanced the binding of Bax alpha to Bcl-2 (Fig. S4), and Asp-33 is central for the activation of Bax by proteases during apoptosis ( ,  ).	bind
50303	5	10710	6	10	NULL	0	NULL	statement 4	NULL		occur during	NULL				apoptosis	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_11_10587_s_251	15590655	A likely explanation for the lack of activity detected with the latter mutant could be that mutation of Lys-64 enhanced the binding of Bax alpha to Bcl-2 (Fig. S4), and Asp-33 is central for the activation of Bax by proteases during apoptosis ( ,  ).	bind
47624	1	10711	5	13	NULL	NULL	NULL	SET7/9	GP		exclude		sterically	residues in lysine binding channel					target lysine side chain with methyl group		NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_177_s_162	12887903	A likely explanation for their different product specificities is that residues in the lysine binding channel of SET7/9 sterically exclude the target lysine side chain with methyl group(s).	bind
46922	1	10711	6	10	NULL	0	NULL	SET7/9	NULL		exclude	NULL	sterically	residues in  lysine binding channel			NULL		lysine side chain with methyl group		NULL		NULL	NULL	NULL	NULL	gw60_molcell_12_1_177_s_162	12887903	A likely explanation for their different product specificities is that residues in the lysine binding channel of SET7/9 sterically exclude the target lysine side chain with methyl group(s).	bind
47625	1	10712	5	13	NULL	NULL	NULL	EcRE1	GP		bind					20E-EcRB11USPP1 complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_7_4897_s_281	10373539	A likely explanation for these findings is that the EcRE1 binds the 20E-EcRB11USPP1 complex, and EcRE-like sequences 2 and 3 bind other transcription factors present in the cell extract.	bind
46923	1	10712	6	NULL	NULL	0	NULL	EcRE1 	NULL		bind	NULL				20E-EcRB11USPP1 complex	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_7_4897_s_281	10373539	A likely explanation for these findings is that the EcRE1 binds the 20E-EcRB11USPP1 complex, and EcRE-like sequences 2 and 3 bind other transcription factors present in the cell extract.	bind
47626	1	10713	5	13	NULL	NULL	NULL	dIgA	GP		bind					pIgR	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_7_1787_s_46	9658171	A likely explanation for these results is that binding of dIgA to the pIgR leads to activation of a phosphatidyl inositol-specific phospholipase C (PLC).	bind
47627	2	10713	5	13	NULL	NULL	NULL	statement 1	Process		leads to					PLC	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_7_1787_s_46	9658171	A likely explanation for these results is that binding of dIgA to the pIgR leads to activation of a phosphatidyl inositol-specific phospholipase C (PLC).	bind
47628	3	10713	5	13	NULL	NULL	NULL	PLC	GP		is					phosphatidyl inositol-specific phospholipase C	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_7_1787_s_46	9658171	A likely explanation for these results is that binding of dIgA to the pIgR leads to activation of a phosphatidyl inositol-specific phospholipase C (PLC).	bind
46924	1	10713	6	NULL	NULL	0	NULL	dIgA	NULL		bind	NULL				pIgR	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_9_7_1787_s_46	9658171	A likely explanation for these results is that binding of dIgA to the pIgR leads to activation of a phosphatidyl inositol-specific phospholipase C (PLC).	bind
46925	2	10713	6	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				PLC	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_9_7_1787_s_46	9658171	A likely explanation for these results is that binding of dIgA to the pIgR leads to activation of a phosphatidyl inositol-specific phospholipase C (PLC).	bind
46926	3	10713	6	NULL	NULL	0	NULL	PLC	NULL		is	NULL				phosphatidyl inositol-specific phospholipase C	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_9_7_1787_s_46	9658171	A likely explanation for these results is that binding of dIgA to the pIgR leads to activation of a phosphatidyl inositol-specific phospholipase C (PLC).	bind
47629	1	10714	5	13	NULL	NULL	NULL	H-NS	GP		bind					donor DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_18_2224_s_270	16166383	A likely explanation for this apparent paradox, and supported by data presented here, is that H-NS binding to the donor DNA initiates unfolding, and then additional molecules of H-NS bind within the terminal inverted repeat, effectively locking in the unfolded conformation.	bind
47630	2	10714	5	13	NULL	NULL	NULL	statement 1	Process		initiates					unfolding	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_18_2224_s_270	16166383	A likely explanation for this apparent paradox, and supported by data presented here, is that H-NS binding to the donor DNA initiates unfolding, and then additional molecules of H-NS bind within the terminal inverted repeat, effectively locking in the unfolded conformation.	bind
47631	3	10714	5	13	NULL	NULL	NULL	H-NS	GP		bind									terminal inverted repeat	NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_18_2224_s_270	16166383	A likely explanation for this apparent paradox, and supported by data presented here, is that H-NS binding to the donor DNA initiates unfolding, and then additional molecules of H-NS bind within the terminal inverted repeat, effectively locking in the unfolded conformation.	bind
47632	4	10714	5	13	NULL	NULL	NULL	statement 3	Process		locks		effectively			unfolded conformation	Process				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_18_2224_s_270	16166383	A likely explanation for this apparent paradox, and supported by data presented here, is that H-NS binding to the donor DNA initiates unfolding, and then additional molecules of H-NS bind within the terminal inverted repeat, effectively locking in the unfolded conformation.	bind
46927	1	10714	6	NULL	NULL	0	NULL	H-NS	NULL		bind	NULL				donor DNA	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_18_2224_s_270	16166383	A likely explanation for this apparent paradox, and supported by data presented here, is that H-NS binding to the donor DNA initiates unfolding, and then additional molecules of H-NS bind within the terminal inverted repeat, effectively locking in the unfolded conformation.	bind
46928	2	10714	6	NULL	NULL	0	NULL	statement 1	NULL		initiates	NULL				unfolding	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_18_2224_s_270	16166383	A likely explanation for this apparent paradox, and supported by data presented here, is that H-NS binding to the donor DNA initiates unfolding, and then additional molecules of H-NS bind within the terminal inverted repeat, effectively locking in the unfolded conformation.	bind
46929	3	10714	6	NULL	NULL	0	NULL	H-NS molecules	NULL		bind	NULL					NULL			terminal inverted repeat	NULL		0	NULL	NULL	NULL	gw70_genesdev_19_18_2224_s_270	16166383	A likely explanation for this apparent paradox, and supported by data presented here, is that H-NS binding to the donor DNA initiates unfolding, and then additional molecules of H-NS bind within the terminal inverted repeat, effectively locking in the unfolded conformation.	bind
50338	4	10714	6	10	NULL	0	NULL	statement 3	NULL		locks	NULL	effectively			unfolded conformation	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_18_2224_s_270	16166383	A likely explanation for this apparent paradox, and supported by data presented here, is that H-NS binding to the donor DNA initiates unfolding, and then additional molecules of H-NS bind within the terminal inverted repeat, effectively locking in the unfolded conformation.	bind
47633	1	10715	5	13	NULL	NULL	NULL	Src protein	GP		bind					PTP1B	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_26_24857_s_206	15866871	A likely explanation for this phenomenon is that Src proteins bound to PTP1B-trapping mutants are catalytically inactive because Tyr527 is phosphorylated, while Src proteins associated with the wild-type PTP1B are activated because of the removal of the inhibitory phosphate.	bind
47634	2	10715	5	13	NULL	NULL	NULL	Src proteins	GP		associate with					PTP1B	GP	wild-type			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_26_24857_s_206	15866871	A likely explanation for this phenomenon is that Src proteins bound to PTP1B-trapping mutants are catalytically inactive because Tyr527 is phosphorylated, while Src proteins associated with the wild-type PTP1B are activated because of the removal of the inhibitory phosphate.	bind
47635	3	10715	5	13	NULL	NULL	NULL	inhibitory phosphate	Chemical	removal of	makes					statement 2	Process	activated			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_26_24857_s_206	15866871	A likely explanation for this phenomenon is that Src proteins bound to PTP1B-trapping mutants are catalytically inactive because Tyr527 is phosphorylated, while Src proteins associated with the wild-type PTP1B are activated because of the removal of the inhibitory phosphate.	bind
47636	4	10715	5	13	NULL	NULL	NULL	Src protein	GP	phosphorylated	makes			Tyr527		statement 1	Process	catalytically inactive			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_26_24857_s_206	15866871	A likely explanation for this phenomenon is that Src proteins bound to PTP1B-trapping mutants are catalytically inactive because Tyr527 is phosphorylated, while Src proteins associated with the wild-type PTP1B are activated because of the removal of the inhibitory phosphate.	bind
46930	1	10715	6	NULL	NULL	0	NULL	Src protein	NULL		bind	NULL				PTP1B	NULL	mutant			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_26_24857_s_206	15866871	A likely explanation for this phenomenon is that Src proteins bound to PTP1B-trapping mutants are catalytically inactive because Tyr527 is phosphorylated, while Src proteins associated with the wild-type PTP1B are activated because of the removal of the inhibitory phosphate.	bind
46931	2	10715	6	NULL	NULL	0	NULL		NULL	phosphorylated	makes	NULL		Tyr527		Src	NULL	catalytically inactive			NULL	statement 1	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_26_24857_s_206	15866871	A likely explanation for this phenomenon is that Src proteins bound to PTP1B-trapping mutants are catalytically inactive because Tyr527 is phosphorylated, while Src proteins associated with the wild-type PTP1B are activated because of the removal of the inhibitory phosphate.	bind
46932	3	10715	6	NULL	NULL	0	NULL	Src protein	NULL		bind	NULL				PTP1B	NULL	wild type			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_26_24857_s_206	15866871	A likely explanation for this phenomenon is that Src proteins bound to PTP1B-trapping mutants are catalytically inactive because Tyr527 is phosphorylated, while Src proteins associated with the wild-type PTP1B are activated because of the removal of the inhibitory phosphate.	bind
46933	4	10715	6	NULL	NULL	0	NULL	phosphate	NULL	removal of;; inhibitory	makes	NULL				Src	NULL	active			NULL	statement 1	0	NULL	NULL	NULL	gw70_jbiolchem_280_26_24857_s_206	15866871	A likely explanation for this phenomenon is that Src proteins bound to PTP1B-trapping mutants are catalytically inactive because Tyr527 is phosphorylated, while Src proteins associated with the wild-type PTP1B are activated because of the removal of the inhibitory phosphate.	bind
47637	1	10717	5	13	NULL	NULL	NULL	IFNAR1/IFNAR2	GP		is a type of					membrane-anchored receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_11_6138_s_229	11344274	A likely explanation is that the  Kd of the soluble receptor for IFN-tau4 (70 nM) is sufficient for it to be detected in a binding assay but too high for it to compete effectively for ligand with the IFNAR1/IFNAR2 membrane-anchored receptor of MDBK cells, which binds IFN-tau with a  Kd of  0.3 nM (unpublished data).	bind
47638	2	10717	5	13	NULL	NULL	NULL	IFNAR1/IFNAR2	GP		bind					IFN-tau	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_11_6138_s_229	11344274	A likely explanation is that the  Kd of the soluble receptor for IFN-tau4 (70 nM) is sufficient for it to be detected in a binding assay but too high for it to compete effectively for ligand with the IFNAR1/IFNAR2 membrane-anchored receptor of MDBK cells, which binds IFN-tau with a  Kd of  0.3 nM (unpublished data).	bind
46934	1	10717	6	NULL	NULL	0	NULL	IFNAR1/IFNAR2	NULL		bind	NULL				IFN-tau	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_98_11_6138_s_229	11344274	A likely explanation is that the  Kd of the soluble receptor for IFN-tau4 (70 nM) is sufficient for it to be detected in a binding assay but too high for it to compete effectively for ligand with the IFNAR1/IFNAR2 membrane-anchored receptor of MDBK cells, which binds IFN-tau with a  Kd of  0.3 nM (unpublished data).	bind
46935	2	10717	6	NULL	NULL	0	NULL	IFNAR1/IFNAR2	NULL		is a type of 	NULL				membrane anchored receptor of MDBK cells	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_98_11_6138_s_229	11344274	A likely explanation is that the  Kd of the soluble receptor for IFN-tau4 (70 nM) is sufficient for it to be detected in a binding assay but too high for it to compete effectively for ligand with the IFNAR1/IFNAR2 membrane-anchored receptor of MDBK cells, which binds IFN-tau with a  Kd of  0.3 nM (unpublished data).	bind
47639	1	10718	5	13	NULL	NULL	NULL	phosphorylation	Process		inhibit		possibly			protein 4.1	GP	function of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_51_47869_s_234	11604393	A likely explanation is the inhibition of protein 4.1 function by phosphorylation, which reduces its ability to promote binding of F-actin to spectrin ( 40,  41).	bind
47640	2	10718	5	13	NULL	NULL	NULL	F-actin	GP		bind					spectrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_51_47869_s_234	11604393	A likely explanation is the inhibition of protein 4.1 function by phosphorylation, which reduces its ability to promote binding of F-actin to spectrin ( 40,  41).	bind
47641	3	10718	5	13	NULL	NULL	NULL	protein 4.1	GP		promotes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_51_47869_s_234	11604393	A likely explanation is the inhibition of protein 4.1 function by phosphorylation, which reduces its ability to promote binding of F-actin to spectrin ( 40,  41).	bind
47642	4	10718	5	13	NULL	NULL	NULL	statement 1	Process		reduces					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_51_47869_s_234	11604393	A likely explanation is the inhibition of protein 4.1 function by phosphorylation, which reduces its ability to promote binding of F-actin to spectrin ( 40,  41).	bind
46936	1	10718	6	NULL	NULL	0	NULL	F-actin	NULL		bind	NULL				spectrin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_51_47869_s_234	11604393	A likely explanation is the inhibition of protein 4.1 function by phosphorylation, which reduces its ability to promote binding of F-actin to spectrin ( 40,  41).	bind
46937	2	10718	6	NULL	NULL	0	NULL	protein 4.1	NULL	function of	is inhibited by	NULL				phosphorylation	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_51_47869_s_234	11604393	A likely explanation is the inhibition of protein 4.1 function by phosphorylation, which reduces its ability to promote binding of F-actin to spectrin ( 40,  41).	bind
46938	3	10718	6	NULL	NULL	0	NULL	protein 4.1	NULL		promotes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_51_47869_s_234	11604393	A likely explanation is the inhibition of protein 4.1 function by phosphorylation, which reduces its ability to promote binding of F-actin to spectrin ( 40,  41).	bind
46939	4	10718	6	NULL	NULL	0	NULL	statement 2	NULL		reduces	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_51_47869_s_234	11604393	A likely explanation is the inhibition of protein 4.1 function by phosphorylation, which reduces its ability to promote binding of F-actin to spectrin ( 40,  41).	bind
47643	1	10719	5	13	NULL	NULL	NULL	JIP-1	GP		bind					APP	GP				NULL		NULL	NULL	NULL	NULL	gw70_jneurosci_25_15_3741_s_368	15829626	A likely explanation, supported by our results ( Fig. 3), is that JIP-1 binding to APP is competed off by proteins with higher affinity or more abundant than JIP-1 (e.g., Fe65) (Matsuda et al., 2001 ), or that in neurons, the phosphorylation of APP through the JIP-3-dependent pathway prevails and is distinct from that implicating JIP-1.	bind
47644	2	10719	5	13	NULL	NULL	NULL	APP	GP	phosphorylation of	occurs through					JIP-3-dependent pathway	Process				NULL	neurons	NULL	NULL	NULL	NULL	gw70_jneurosci_25_15_3741_s_368	15829626	A likely explanation, supported by our results ( Fig. 3), is that JIP-1 binding to APP is competed off by proteins with higher affinity or more abundant than JIP-1 (e.g., Fe65) (Matsuda et al., 2001 ), or that in neurons, the phosphorylation of APP through the JIP-3-dependent pathway prevails and is distinct from that implicating JIP-1.	bind
46940	1	10719	6	NULL	NULL	0	NULL	JIP-1	NULL		bind	NULL				APP	NULL				NULL		0	NULL	NULL	NULL	gw70_jneurosci_25_15_3741_s_368	15829626	A likely explanation, supported by our results ( Fig. 3), is that JIP-1 binding to APP is competed off by proteins with higher affinity or more abundant than JIP-1 (e.g., Fe65) (Matsuda et al., 2001 ), or that in neurons, the phosphorylation of APP through the JIP-3-dependent pathway prevails and is distinct from that implicating JIP-1.	bind
46941	2	10719	6	NULL	NULL	0	NULL	APP	NULL	phosphorylation of	occurs through	NULL				JIP-3-dependent pathway	NULL				NULL	neurons	NULL	NULL	NULL	NULL	gw70_jneurosci_25_15_3741_s_368	15829626	A likely explanation, supported by our results ( Fig. 3), is that JIP-1 binding to APP is competed off by proteins with higher affinity or more abundant than JIP-1 (e.g., Fe65) (Matsuda et al., 2001 ), or that in neurons, the phosphorylation of APP through the JIP-3-dependent pathway prevails and is distinct from that implicating JIP-1.	bind
47645	1	10720	5	13	NULL	NULL	NULL	regulatory proteins	GP		bind								terminal alpha rings		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_24_18557_s_27	10764772	A likely mechanism for control of substrate access to the proteasome involves binding of regulatory proteins to its terminal alpha rings.	bind
50342	2	10720	5	13	NULL	NULL	NULL	substrate	GP		access to					proteasome	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_24_18557_s_27	10764772	A likely mechanism for control of substrate access to the proteasome involves binding of regulatory proteins to its terminal alpha rings.	bind
50343	3	10720	5	13	NULL	NULL	NULL	statement 2	Process	control of	involves					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_24_18557_s_27	10764772	A likely mechanism for control of substrate access to the proteasome involves binding of regulatory proteins to its terminal alpha rings.	bind
46942	1	10720	6	10	NULL	0	NULL	regulatory proteins	NULL		bind	NULL				alpha rings	NULL		terminal		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_24_18557_s_27	10764772	A likely mechanism for control of substrate access to the proteasome involves binding of regulatory proteins to its terminal alpha rings.	bind
46973	2	10720	6	NULL	NULL	0	NULL	substrate	NULL		access to	NULL				proteasome	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_24_18557_s_27	10764772	A likely mechanism for control of substrate access to the proteasome involves binding of regulatory proteins to its terminal alpha rings.	bind
46974	3	10720	6	NULL	NULL	0	NULL	statement 2	NULL	control of	involves	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_24_18557_s_27	10764772	A likely mechanism for control of substrate access to the proteasome involves binding of regulatory proteins to its terminal alpha rings.	bind
50802	1	10721	5	13	NULL	NULL	NULL	Abeta	GP		is present in					membrane compartment	CellComponent	detergent-insoluble			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_36_27901_s_27	10846187	A likely possibility is that the earliest abnormality in beta-amyloidogenesis is the altered intracellular trafficking of the specific membrane domains, because i) a substantial fraction of Abeta is present in the detergent-insoluble membrane compartment, which is rich in cholesterol and sphingolipids, in cultured cells and rat brains ( 26,  27); ii) Abeta, generated from apically missorted APP in a cholesterol-dependent manner in Madin-Darby canine kidney cells, serves as a seed for Abeta fibrillogenesis ( 28); iii) GM1 ganglioside-bound Abeta is detected in Down's syndrome brains exhibiting exclusively diffuse plaques, the earliest stage of senile plaques ( 29); and iv) the addition of GM1-containing vesicles to Abeta solution dramatically accelerates Abeta fibril formation  in vitro ( 30).	bind
50803	2	10721	5	13	NULL	NULL	NULL	membrane compartment	CellComponent	detergent-insoluble	is rich in					cholesterol	Chemical				NULL	cultured cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_36_27901_s_27	10846187	A likely possibility is that the earliest abnormality in beta-amyloidogenesis is the altered intracellular trafficking of the specific membrane domains, because i) a substantial fraction of Abeta is present in the detergent-insoluble membrane compartment, which is rich in cholesterol and sphingolipids, in cultured cells and rat brains ( 26,  27); ii) Abeta, generated from apically missorted APP in a cholesterol-dependent manner in Madin-Darby canine kidney cells, serves as a seed for Abeta fibrillogenesis ( 28); iii) GM1 ganglioside-bound Abeta is detected in Down's syndrome brains exhibiting exclusively diffuse plaques, the earliest stage of senile plaques ( 29); and iv) the addition of GM1-containing vesicles to Abeta solution dramatically accelerates Abeta fibril formation  in vitro ( 30).	bind
50804	3	10721	5	13	NULL	NULL	NULL	membrane compartment	CellComponent	detergent-insoluble	is rich in					sphingolipids	Chemical				NULL	cultured cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_36_27901_s_27	10846187	A likely possibility is that the earliest abnormality in beta-amyloidogenesis is the altered intracellular trafficking of the specific membrane domains, because i) a substantial fraction of Abeta is present in the detergent-insoluble membrane compartment, which is rich in cholesterol and sphingolipids, in cultured cells and rat brains ( 26,  27); ii) Abeta, generated from apically missorted APP in a cholesterol-dependent manner in Madin-Darby canine kidney cells, serves as a seed for Abeta fibrillogenesis ( 28); iii) GM1 ganglioside-bound Abeta is detected in Down's syndrome brains exhibiting exclusively diffuse plaques, the earliest stage of senile plaques ( 29); and iv) the addition of GM1-containing vesicles to Abeta solution dramatically accelerates Abeta fibril formation  in vitro ( 30).	bind
50805	4	10721	5	13	NULL	NULL	NULL	membrane compartment	CellComponent	detergent-insoluble	is rich in					cholesterol	Chemical				NULL	rat brains	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_36_27901_s_27	10846187	A likely possibility is that the earliest abnormality in beta-amyloidogenesis is the altered intracellular trafficking of the specific membrane domains, because i) a substantial fraction of Abeta is present in the detergent-insoluble membrane compartment, which is rich in cholesterol and sphingolipids, in cultured cells and rat brains ( 26,  27); ii) Abeta, generated from apically missorted APP in a cholesterol-dependent manner in Madin-Darby canine kidney cells, serves as a seed for Abeta fibrillogenesis ( 28); iii) GM1 ganglioside-bound Abeta is detected in Down's syndrome brains exhibiting exclusively diffuse plaques, the earliest stage of senile plaques ( 29); and iv) the addition of GM1-containing vesicles to Abeta solution dramatically accelerates Abeta fibril formation  in vitro ( 30).	bind
50806	5	10721	5	13	NULL	NULL	NULL	membrane compartment	CellComponent	detergent-insoluble	is rich in					sphingolipids	Chemical				NULL	rat brains	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_36_27901_s_27	10846187	A likely possibility is that the earliest abnormality in beta-amyloidogenesis is the altered intracellular trafficking of the specific membrane domains, because i) a substantial fraction of Abeta is present in the detergent-insoluble membrane compartment, which is rich in cholesterol and sphingolipids, in cultured cells and rat brains ( 26,  27); ii) Abeta, generated from apically missorted APP in a cholesterol-dependent manner in Madin-Darby canine kidney cells, serves as a seed for Abeta fibrillogenesis ( 28); iii) GM1 ganglioside-bound Abeta is detected in Down's syndrome brains exhibiting exclusively diffuse plaques, the earliest stage of senile plaques ( 29); and iv) the addition of GM1-containing vesicles to Abeta solution dramatically accelerates Abeta fibril formation  in vitro ( 30).	bind
50807	6	10721	5	13	NULL	NULL	NULL	Abeta	GP		is generated from					APP	GP	apically missorted			NULL	Madin-Darby canine kidney cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_36_27901_s_27	10846187	A likely possibility is that the earliest abnormality in beta-amyloidogenesis is the altered intracellular trafficking of the specific membrane domains, because i) a substantial fraction of Abeta is present in the detergent-insoluble membrane compartment, which is rich in cholesterol and sphingolipids, in cultured cells and rat brains ( 26,  27); ii) Abeta, generated from apically missorted APP in a cholesterol-dependent manner in Madin-Darby canine kidney cells, serves as a seed for Abeta fibrillogenesis ( 28); iii) GM1 ganglioside-bound Abeta is detected in Down's syndrome brains exhibiting exclusively diffuse plaques, the earliest stage of senile plaques ( 29); and iv) the addition of GM1-containing vesicles to Abeta solution dramatically accelerates Abeta fibril formation  in vitro ( 30).	bind
50808	7	10721	5	13	NULL	NULL	NULL	statement 6	Process		is dependent on					cholesterol	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_36_27901_s_27	10846187	A likely possibility is that the earliest abnormality in beta-amyloidogenesis is the altered intracellular trafficking of the specific membrane domains, because i) a substantial fraction of Abeta is present in the detergent-insoluble membrane compartment, which is rich in cholesterol and sphingolipids, in cultured cells and rat brains ( 26,  27); ii) Abeta, generated from apically missorted APP in a cholesterol-dependent manner in Madin-Darby canine kidney cells, serves as a seed for Abeta fibrillogenesis ( 28); iii) GM1 ganglioside-bound Abeta is detected in Down's syndrome brains exhibiting exclusively diffuse plaques, the earliest stage of senile plaques ( 29); and iv) the addition of GM1-containing vesicles to Abeta solution dramatically accelerates Abeta fibril formation  in vitro ( 30).	bind
50809	8	10721	5	13	NULL	NULL	NULL	statement 6	Process		serves as a seed for					Abeta fibrillogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_36_27901_s_27	10846187	A likely possibility is that the earliest abnormality in beta-amyloidogenesis is the altered intracellular trafficking of the specific membrane domains, because i) a substantial fraction of Abeta is present in the detergent-insoluble membrane compartment, which is rich in cholesterol and sphingolipids, in cultured cells and rat brains ( 26,  27); ii) Abeta, generated from apically missorted APP in a cholesterol-dependent manner in Madin-Darby canine kidney cells, serves as a seed for Abeta fibrillogenesis ( 28); iii) GM1 ganglioside-bound Abeta is detected in Down's syndrome brains exhibiting exclusively diffuse plaques, the earliest stage of senile plaques ( 29); and iv) the addition of GM1-containing vesicles to Abeta solution dramatically accelerates Abeta fibril formation  in vitro ( 30).	bind
50810	9	10721	5	13	NULL	NULL	NULL	GM1 ganglioside	GP		bind					Abeta	GP				NULL	Down's syndrome brains exhibiting exclusively diffuse plaques	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_36_27901_s_27	10846187	A likely possibility is that the earliest abnormality in beta-amyloidogenesis is the altered intracellular trafficking of the specific membrane domains, because i) a substantial fraction of Abeta is present in the detergent-insoluble membrane compartment, which is rich in cholesterol and sphingolipids, in cultured cells and rat brains ( 26,  27); ii) Abeta, generated from apically missorted APP in a cholesterol-dependent manner in Madin-Darby canine kidney cells, serves as a seed for Abeta fibrillogenesis ( 28); iii) GM1 ganglioside-bound Abeta is detected in Down's syndrome brains exhibiting exclusively diffuse plaques, the earliest stage of senile plaques ( 29); and iv) the addition of GM1-containing vesicles to Abeta solution dramatically accelerates Abeta fibril formation  in vitro ( 30).	bind
50811	10	10721	5	13	NULL	NULL	NULL	GM1-containing vesicles	CellComponent		accelerates		dramatically			Abeta	GP	fibril formation of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_36_27901_s_27	10846187	A likely possibility is that the earliest abnormality in beta-amyloidogenesis is the altered intracellular trafficking of the specific membrane domains, because i) a substantial fraction of Abeta is present in the detergent-insoluble membrane compartment, which is rich in cholesterol and sphingolipids, in cultured cells and rat brains ( 26,  27); ii) Abeta, generated from apically missorted APP in a cholesterol-dependent manner in Madin-Darby canine kidney cells, serves as a seed for Abeta fibrillogenesis ( 28); iii) GM1 ganglioside-bound Abeta is detected in Down's syndrome brains exhibiting exclusively diffuse plaques, the earliest stage of senile plaques ( 29); and iv) the addition of GM1-containing vesicles to Abeta solution dramatically accelerates Abeta fibril formation  in vitro ( 30).	bind
47371	1	10721	6	NULL	NULL	0	NULL	Abeta	NULL		is present in	NULL				membrane compartment	NULL	detergent insoluble			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_36_27901_s_27	10846187	A likely possibility is that the earliest abnormality in beta-amyloidogenesis is the altered intracellular trafficking of the specific membrane domains, because i) a substantial fraction of Abeta is present in the detergent-insoluble membrane compartment, which is rich in cholesterol and sphingolipids, in cultured cells and rat brains ( 26,  27); ii) Abeta, generated from apically missorted APP in a cholesterol-dependent manner in Madin-Darby canine kidney cells, serves as a seed for Abeta fibrillogenesis ( 28); iii) GM1 ganglioside-bound Abeta is detected in Down's syndrome brains exhibiting exclusively diffuse plaques, the earliest stage of senile plaques ( 29); and iv) the addition of GM1-containing vesicles to Abeta solution dramatically accelerates Abeta fibril formation  in vitro ( 30).	bind
47372	2	10721	6	NULL	NULL	0	NULL	membrane compartment	NULL	detergent insoluble	is rich in	NULL				cholesterol	NULL				NULL	cultured cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_36_27901_s_27	10846187	A likely possibility is that the earliest abnormality in beta-amyloidogenesis is the altered intracellular trafficking of the specific membrane domains, because i) a substantial fraction of Abeta is present in the detergent-insoluble membrane compartment, which is rich in cholesterol and sphingolipids, in cultured cells and rat brains ( 26,  27); ii) Abeta, generated from apically missorted APP in a cholesterol-dependent manner in Madin-Darby canine kidney cells, serves as a seed for Abeta fibrillogenesis ( 28); iii) GM1 ganglioside-bound Abeta is detected in Down's syndrome brains exhibiting exclusively diffuse plaques, the earliest stage of senile plaques ( 29); and iv) the addition of GM1-containing vesicles to Abeta solution dramatically accelerates Abeta fibril formation  in vitro ( 30).	bind
47373	3	10721	6	NULL	NULL	0	NULL	membrane compartment	NULL	detergent insoluble	is rich in	NULL				sphingolipids	NULL				NULL	cultured cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_36_27901_s_27	10846187	A likely possibility is that the earliest abnormality in beta-amyloidogenesis is the altered intracellular trafficking of the specific membrane domains, because i) a substantial fraction of Abeta is present in the detergent-insoluble membrane compartment, which is rich in cholesterol and sphingolipids, in cultured cells and rat brains ( 26,  27); ii) Abeta, generated from apically missorted APP in a cholesterol-dependent manner in Madin-Darby canine kidney cells, serves as a seed for Abeta fibrillogenesis ( 28); iii) GM1 ganglioside-bound Abeta is detected in Down's syndrome brains exhibiting exclusively diffuse plaques, the earliest stage of senile plaques ( 29); and iv) the addition of GM1-containing vesicles to Abeta solution dramatically accelerates Abeta fibril formation  in vitro ( 30).	bind
47374	4	10721	6	NULL	NULL	0	NULL	membrane compartment	NULL	detergent insoluble	is rich in	NULL				cholesterol	NULL				NULL	rat brains	0	NULL	NULL	NULL	gw60_jbiolchem_275_36_27901_s_27	10846187	A likely possibility is that the earliest abnormality in beta-amyloidogenesis is the altered intracellular trafficking of the specific membrane domains, because i) a substantial fraction of Abeta is present in the detergent-insoluble membrane compartment, which is rich in cholesterol and sphingolipids, in cultured cells and rat brains ( 26,  27); ii) Abeta, generated from apically missorted APP in a cholesterol-dependent manner in Madin-Darby canine kidney cells, serves as a seed for Abeta fibrillogenesis ( 28); iii) GM1 ganglioside-bound Abeta is detected in Down's syndrome brains exhibiting exclusively diffuse plaques, the earliest stage of senile plaques ( 29); and iv) the addition of GM1-containing vesicles to Abeta solution dramatically accelerates Abeta fibril formation  in vitro ( 30).	bind
47375	5	10721	6	NULL	NULL	0	NULL	membrane compartment	NULL	detergent insoluble	is rich in	NULL				sphingolipids	NULL				NULL	rat brains	0	NULL	NULL	NULL	gw60_jbiolchem_275_36_27901_s_27	10846187	A likely possibility is that the earliest abnormality in beta-amyloidogenesis is the altered intracellular trafficking of the specific membrane domains, because i) a substantial fraction of Abeta is present in the detergent-insoluble membrane compartment, which is rich in cholesterol and sphingolipids, in cultured cells and rat brains ( 26,  27); ii) Abeta, generated from apically missorted APP in a cholesterol-dependent manner in Madin-Darby canine kidney cells, serves as a seed for Abeta fibrillogenesis ( 28); iii) GM1 ganglioside-bound Abeta is detected in Down's syndrome brains exhibiting exclusively diffuse plaques, the earliest stage of senile plaques ( 29); and iv) the addition of GM1-containing vesicles to Abeta solution dramatically accelerates Abeta fibril formation  in vitro ( 30).	bind
47376	6	10721	6	NULL	NULL	0	NULL	APP	NULL	apically missorted	serves as a seed for	NULL				Abeta fibrillogenesis	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_36_27901_s_27	10846187	A likely possibility is that the earliest abnormality in beta-amyloidogenesis is the altered intracellular trafficking of the specific membrane domains, because i) a substantial fraction of Abeta is present in the detergent-insoluble membrane compartment, which is rich in cholesterol and sphingolipids, in cultured cells and rat brains ( 26,  27); ii) Abeta, generated from apically missorted APP in a cholesterol-dependent manner in Madin-Darby canine kidney cells, serves as a seed for Abeta fibrillogenesis ( 28); iii) GM1 ganglioside-bound Abeta is detected in Down's syndrome brains exhibiting exclusively diffuse plaques, the earliest stage of senile plaques ( 29); and iv) the addition of GM1-containing vesicles to Abeta solution dramatically accelerates Abeta fibril formation  in vitro ( 30).	bind
47377	7	10721	6	NULL	NULL	0	NULL	GM1 ganglioside	NULL		bind	NULL				Abeta	NULL				NULL	Down's syndrome brains exhibiting exclusively diffuse plaques	0	NULL	NULL	NULL	gw60_jbiolchem_275_36_27901_s_27	10846187	A likely possibility is that the earliest abnormality in beta-amyloidogenesis is the altered intracellular trafficking of the specific membrane domains, because i) a substantial fraction of Abeta is present in the detergent-insoluble membrane compartment, which is rich in cholesterol and sphingolipids, in cultured cells and rat brains ( 26,  27); ii) Abeta, generated from apically missorted APP in a cholesterol-dependent manner in Madin-Darby canine kidney cells, serves as a seed for Abeta fibrillogenesis ( 28); iii) GM1 ganglioside-bound Abeta is detected in Down's syndrome brains exhibiting exclusively diffuse plaques, the earliest stage of senile plaques ( 29); and iv) the addition of GM1-containing vesicles to Abeta solution dramatically accelerates Abeta fibril formation  in vitro ( 30).	bind
47378	8	10721	6	NULL	NULL	0	NULL	GM1-containing vesicles	NULL	addition of	accelerates	NULL				Abeta	NULL	fibril formation of			NULL	in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_275_36_27901_s_27	10846187	A likely possibility is that the earliest abnormality in beta-amyloidogenesis is the altered intracellular trafficking of the specific membrane domains, because i) a substantial fraction of Abeta is present in the detergent-insoluble membrane compartment, which is rich in cholesterol and sphingolipids, in cultured cells and rat brains ( 26,  27); ii) Abeta, generated from apically missorted APP in a cholesterol-dependent manner in Madin-Darby canine kidney cells, serves as a seed for Abeta fibrillogenesis ( 28); iii) GM1 ganglioside-bound Abeta is detected in Down's syndrome brains exhibiting exclusively diffuse plaques, the earliest stage of senile plaques ( 29); and iv) the addition of GM1-containing vesicles to Abeta solution dramatically accelerates Abeta fibril formation  in vitro ( 30).	bind
47646	1	10722	5	13	NULL	NULL	NULL	AP-1	GP		suppress					ET-1	GP	expression of			NULL	EC	NULL	NULL	NULL	NULL	gw70_circulationres_98_2_192_s_236	16357303	A likely role of BA/FXR-mediated inhibition of AP-1 activity in suppressing ET-1 expression in EC was further supported by results from ChIP assays in which CDCA treatment led to decreased binding of c-Jun to an AP-1 binding site in ET-1 promoter in RPAEC ( Figure 8C).	bind
47647	2	10722	5	13	NULL	NULL	NULL	c-Jun	GP		bind					ET-1	GP			AP-1 binding site in promoter	NULL	RPAEC	NULL	NULL	NULL	NULL	gw70_circulationres_98_2_192_s_236	16357303	A likely role of BA/FXR-mediated inhibition of AP-1 activity in suppressing ET-1 expression in EC was further supported by results from ChIP assays in which CDCA treatment led to decreased binding of c-Jun to an AP-1 binding site in ET-1 promoter in RPAEC ( Figure 8C).	bind
50344	3	10722	5	13	NULL	NULL	NULL	BA/FXR	GP		mediates					statement 1	Process	inhibition of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_2_192_s_236	16357303	A likely role of BA/FXR-mediated inhibition of AP-1 activity in suppressing ET-1 expression in EC was further supported by results from ChIP assays in which CDCA treatment led to decreased binding of c-Jun to an AP-1 binding site in ET-1 promoter in RPAEC ( Figure 8C).	bind
50345	4	10722	5	13	NULL	NULL	NULL	CDCA	GP		decrease					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_98_2_192_s_236	16357303	A likely role of BA/FXR-mediated inhibition of AP-1 activity in suppressing ET-1 expression in EC was further supported by results from ChIP assays in which CDCA treatment led to decreased binding of c-Jun to an AP-1 binding site in ET-1 promoter in RPAEC ( Figure 8C).	bind
46975	1	10722	6	NULL	NULL	0	NULL	c-Jun	NULL		bind	NULL				ET-1	NULL			AP-1 binding site of promoter	NULL		0	NULL	NULL	NULL	gw70_circulationres_98_2_192_s_236	16357303	A likely role of BA/FXR-mediated inhibition of AP-1 activity in suppressing ET-1 expression in EC was further supported by results from ChIP assays in which CDCA treatment led to decreased binding of c-Jun to an AP-1 binding site in ET-1 promoter in RPAEC ( Figure 8C).	bind
46976	2	10722	6	10	NULL	0	NULL	AP-1	NULL		suppress	NULL				ET-1	NULL	expression of			NULL	EC	NULL	NULL	NULL	NULL	gw70_circulationres_98_2_192_s_236	16357303	A likely role of BA/FXR-mediated inhibition of AP-1 activity in suppressing ET-1 expression in EC was further supported by results from ChIP assays in which CDCA treatment led to decreased binding of c-Jun to an AP-1 binding site in ET-1 promoter in RPAEC ( Figure 8C).	bind
46977	3	10722	6	NULL	NULL	0	NULL	CDCA	NULL		decreases	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_2_192_s_236	16357303	A likely role of BA/FXR-mediated inhibition of AP-1 activity in suppressing ET-1 expression in EC was further supported by results from ChIP assays in which CDCA treatment led to decreased binding of c-Jun to an AP-1 binding site in ET-1 promoter in RPAEC ( Figure 8C).	bind
50347	4	10722	6	10	NULL	0	NULL	BA/FXR	NULL		mediates	NULL				statement 2	NULL	inhibition of			NULL		0	NULL	NULL	NULL	gw70_circulationres_98_2_192_s_236	16357303	A likely role of BA/FXR-mediated inhibition of AP-1 activity in suppressing ET-1 expression in EC was further supported by results from ChIP assays in which CDCA treatment led to decreased binding of c-Jun to an AP-1 binding site in ET-1 promoter in RPAEC ( Figure 8C).	bind
47648	1	10723	5	13	NULL	NULL	NULL	SR proteins	GP		bind					exon	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_6_2411_s_139	7852296	A likely scenario invokes interactions between the SR  proteins bound to one exon with the SR proteins bound to an adjoining  exon.	bind
46978	1	10723	6	NULL	NULL	0	NULL	SR protein	NULL		bind	NULL				exon	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_6_2411_s_139	7852296	A likely scenario invokes interactions between the SR  proteins bound to one exon with the SR proteins bound to an adjoining  exon.	bind
47649	1	10725	5	13	NULL	NULL	NULL	PhcA	GP		bind					P xpsR	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbacteriol_180_10_2736_s_216	9573161	A likely site centered around  77 was confirmed and further defined by analysis of the effects of mutations in the site on in vivo expression from P xpsR and in vitro binding of PhcA to P xpsR.	bind
46979	1	10725	6	NULL	NULL	0	NULL	PhcA	NULL		bind	NULL				P xpsR	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_jbacteriol_180_10_2736_s_216	9573161	A likely site centered around  77 was confirmed and further defined by analysis of the effects of mutations in the site on in vivo expression from P xpsR and in vitro binding of PhcA to P xpsR.	bind
47650	1	10726	5	13	NULL	NULL	NULL	FAD	Chemical		bind					AO monomers	GP				NULL	cytosol	NULL	NULL	NULL	NULL	gw60_molbiolcell_14_2_786_s_303	12589070	A likely way to explain both observations is that FAD binding to AO monomers in the cytosol is a prerequisite to allow efficient translocation into peroxisomes.	bind
50348	2	10726	5	13	NULL	NULL	NULL	statement 1	GP		allows					peroxisomes	CellComponent	translocation into			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_14_2_786_s_303	12589070	A likely way to explain both observations is that FAD binding to AO monomers in the cytosol is a prerequisite to allow efficient translocation into peroxisomes.	bind
46980	1	10726	6	NULL	NULL	0	NULL	FAD	NULL		bind	NULL				AO monomers	NULL				NULL	cytosol	0	NULL	NULL	NULL	gw60_molbiolcell_14_2_786_s_303	12589070	A likely way to explain both observations is that FAD binding to AO monomers in the cytosol is a prerequisite to allow efficient translocation into peroxisomes.	bind
46981	2	10726	6	NULL	NULL	0	NULL	statement 1	NULL		allows	NULL				peroxisomes	NULL	translocation into			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_2_786_s_303	12589070	A likely way to explain both observations is that FAD binding to AO monomers in the cytosol is a prerequisite to allow efficient translocation into peroxisomes.	bind
47651	1	10727	5	13	NULL	NULL	NULL	Ajuba protein	GP		bind			LIM domain		Aurora-A	GP	human	N-terminal noncatalytic domain of 		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_45_47201_s_301	15316025	A LIM domain containing the protein Ajuba binds and activates human Aurora-A through the N-terminal noncatalytic domain of Aurora-A ( ).	bind
47652	2	10727	5	13	NULL	NULL	NULL	statement 1	Process		activates					Aurora-A	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_45_47201_s_301	15316025	A LIM domain containing the protein Ajuba binds and activates human Aurora-A through the N-terminal noncatalytic domain of Aurora-A ( ).	bind
46982	1	10727	6	NULL	NULL	0	NULL	Ajuba protein	NULL		bind	NULL		LIM domain		Aurora-A	NULL	human	N-terminal noncatalytic domain		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_45_47201_s_301	15316025	A LIM domain containing the protein Ajuba binds and activates human Aurora-A through the N-terminal noncatalytic domain of Aurora-A ( ).	bind
46983	2	10727	6	10	NULL	0	NULL	statement 1			activates					Aurora-A		human			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_45_47201_s_301	15316025	A LIM domain containing the protein Ajuba binds and activates human Aurora-A through the N-terminal noncatalytic domain of Aurora-A ( ).	bind
47653	1	10728	5	13	NULL	NULL	NULL	Translin/Trax	GP		bind					L-PK	GP			GRE	NULL	in vivo	NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1624_1_29_s_178	14642810	A limitation of our study,  however, is that we do not presently know the extent of Translin/Trax binding to  the L-PK GRE in vivo.	bind
46984	1	10728	6	NULL	NULL	0	NULL	Translin/Trax	NULL		bind	NULL				L-PK	NULL			GRE	NULL	in vivo	0	NULL	NULL	NULL	gw70_biochimbiophysacta_1624_1_29_s_178	14642810	A limitation of our study,  however, is that we do not presently know the extent of Translin/Trax binding to  the L-PK GRE in vivo.	bind
47654	1	10729	5	13	NULL	NULL	NULL	TF	GP		bind					VII variants	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_19875_s_84	9242651	A limitation of the competitive assay approach is the presence of substrate that could differentially affect TF binding by the VII variants.	bind
46985	1	10729	6	NULL	NULL	0	NULL	VII variants	NULL		bind	NULL				TF	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_32_19875_s_84	9242651	A limitation of the competitive assay approach is the presence of substrate that could differentially affect TF binding by the VII variants.	bind
47655	1	10730	5	13	NULL	NULL	NULL	HeLa cells	Cell		contains					RARalpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_8_4355_s_161	8626785	A limitation of these experiments was that  HeLa cells contain multiple retinoid receptors (RARalpha, RAR ,  RXRbeta),   and the ligand used in these studies (ATRA) can  activate both classes of receptors (it binds to RARs directly and can  be isomerized  in vivo  to 9- cis-RA, which binds to  RXRs).	bind
47656	2	10730	5	13	NULL	NULL	NULL	RARalpha	GP		is a type of					retinoid receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_8_4355_s_161	8626785	A limitation of these experiments was that  HeLa cells contain multiple retinoid receptors (RARalpha, RAR ,  RXRbeta),   and the ligand used in these studies (ATRA) can  activate both classes of receptors (it binds to RARs directly and can  be isomerized  in vivo  to 9- cis-RA, which binds to  RXRs).	bind
47657	3	10730	5	13	NULL	NULL	NULL	HeLa cells	Cell		contains					RAR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_8_4355_s_161	8626785	A limitation of these experiments was that  HeLa cells contain multiple retinoid receptors (RARalpha, RAR ,  RXRbeta),   and the ligand used in these studies (ATRA) can  activate both classes of receptors (it binds to RARs directly and can  be isomerized  in vivo  to 9- cis-RA, which binds to  RXRs).	bind
47658	4	10730	5	13	NULL	NULL	NULL	RAR	GP		is a type of					retinoid receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_8_4355_s_161	8626785	A limitation of these experiments was that  HeLa cells contain multiple retinoid receptors (RARalpha, RAR ,  RXRbeta),   and the ligand used in these studies (ATRA) can  activate both classes of receptors (it binds to RARs directly and can  be isomerized  in vivo  to 9- cis-RA, which binds to  RXRs).	bind
47659	5	10730	5	13	NULL	NULL	NULL	HeLa cells	Cell		contains					RXRbeta	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_8_4355_s_161	8626785	A limitation of these experiments was that  HeLa cells contain multiple retinoid receptors (RARalpha, RAR ,  RXRbeta),   and the ligand used in these studies (ATRA) can  activate both classes of receptors (it binds to RARs directly and can  be isomerized  in vivo  to 9- cis-RA, which binds to  RXRs).	bind
47660	6	10730	5	13	NULL	NULL	NULL	RXRbeta	GP		is a type of					retinoid receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_8_4355_s_161	8626785	A limitation of these experiments was that  HeLa cells contain multiple retinoid receptors (RARalpha, RAR ,  RXRbeta),   and the ligand used in these studies (ATRA) can  activate both classes of receptors (it binds to RARs directly and can  be isomerized  in vivo  to 9- cis-RA, which binds to  RXRs).	bind
47661	7	10730	5	13	NULL	NULL	NULL	ATRA ligand	GP		bind		directly			RARs	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_8_4355_s_161	8626785	A limitation of these experiments was that  HeLa cells contain multiple retinoid receptors (RARalpha, RAR ,  RXRbeta),   and the ligand used in these studies (ATRA) can  activate both classes of receptors (it binds to RARs directly and can  be isomerized  in vivo  to 9- cis-RA, which binds to  RXRs).	bind
47662	8	10730	5	13	NULL	NULL	NULL	ATRA ligand	GP		is isomerized to					9- cis-RA	Chemical				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_8_4355_s_161	8626785	A limitation of these experiments was that  HeLa cells contain multiple retinoid receptors (RARalpha, RAR ,  RXRbeta),   and the ligand used in these studies (ATRA) can  activate both classes of receptors (it binds to RARs directly and can  be isomerized  in vivo  to 9- cis-RA, which binds to  RXRs).	bind
47663	9	10730	5	13	NULL	NULL	NULL	9- cis-RA	Chemical		bind					RXRs	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_8_4355_s_161	8626785	A limitation of these experiments was that  HeLa cells contain multiple retinoid receptors (RARalpha, RAR ,  RXRbeta),   and the ligand used in these studies (ATRA) can  activate both classes of receptors (it binds to RARs directly and can  be isomerized  in vivo  to 9- cis-RA, which binds to  RXRs).	bind
46986	1	10730	6	NULL	NULL	0	NULL	HeLa cells	NULL		contains	NULL				RARalpha	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_8_4355_s_161	8626785	A limitation of these experiments was that  HeLa cells contain multiple retinoid receptors (RARalpha, RAR ,  RXRbeta),   and the ligand used in these studies (ATRA) can  activate both classes of receptors (it binds to RARs directly and can  be isomerized  in vivo  to 9- cis-RA, which binds to  RXRs).	bind
46987	2	10730	6	NULL	NULL	0	NULL	HeLa cells	NULL		contain	NULL				RAR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_8_4355_s_161	8626785	A limitation of these experiments was that  HeLa cells contain multiple retinoid receptors (RARalpha, RAR ,  RXRbeta),   and the ligand used in these studies (ATRA) can  activate both classes of receptors (it binds to RARs directly and can  be isomerized  in vivo  to 9- cis-RA, which binds to  RXRs).	bind
46988	3	10730	6	NULL	NULL	0	NULL	HeLa cells	NULL		contain	NULL				RXRbeta	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_8_4355_s_161	8626785	A limitation of these experiments was that  HeLa cells contain multiple retinoid receptors (RARalpha, RAR ,  RXRbeta),   and the ligand used in these studies (ATRA) can  activate both classes of receptors (it binds to RARs directly and can  be isomerized  in vivo  to 9- cis-RA, which binds to  RXRs).	bind
46989	4	10730	6	NULL	NULL	0	NULL	ATRA	NULL		bind	NULL	directly			RARs	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_8_4355_s_161	8626785	A limitation of these experiments was that  HeLa cells contain multiple retinoid receptors (RARalpha, RAR ,  RXRbeta),   and the ligand used in these studies (ATRA) can  activate both classes of receptors (it binds to RARs directly and can  be isomerized  in vivo  to 9- cis-RA, which binds to  RXRs).	bind
46990	5	10730	6	NULL	NULL	0	NULL	ATRA	NULL		is isomerized to	NULL				9- cis-RA	NULL				NULL	in vivo	0	NULL	NULL	NULL	gw60_jbiolchem_271_8_4355_s_161	8626785	A limitation of these experiments was that  HeLa cells contain multiple retinoid receptors (RARalpha, RAR ,  RXRbeta),   and the ligand used in these studies (ATRA) can  activate both classes of receptors (it binds to RARs directly and can  be isomerized  in vivo  to 9- cis-RA, which binds to  RXRs).	bind
46991	6	10730	6	NULL	NULL	0	NULL	9- cis-RA	NULL		bind	NULL				RXRs	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_8_4355_s_161	8626785	A limitation of these experiments was that  HeLa cells contain multiple retinoid receptors (RARalpha, RAR ,  RXRbeta),   and the ligand used in these studies (ATRA) can  activate both classes of receptors (it binds to RARs directly and can  be isomerized  in vivo  to 9- cis-RA, which binds to  RXRs).	bind
50349	7	10730	6	10	NULL	0	NULL	RARalpha	NULL		is a type of	NULL				retinoid receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_8_4355_s_161	8626785	A limitation of these experiments was that  HeLa cells contain multiple retinoid receptors (RARalpha, RAR ,  RXRbeta),   and the ligand used in these studies (ATRA) can  activate both classes of receptors (it binds to RARs directly and can  be isomerized  in vivo  to 9- cis-RA, which binds to  RXRs).	bind
50350	8	10730	6	10	NULL	0	NULL	RAR	NULL		is a type of	NULL				retinoid receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_8_4355_s_161	8626785	A limitation of these experiments was that  HeLa cells contain multiple retinoid receptors (RARalpha, RAR ,  RXRbeta),   and the ligand used in these studies (ATRA) can  activate both classes of receptors (it binds to RARs directly and can  be isomerized  in vivo  to 9- cis-RA, which binds to  RXRs).	bind
50351	9	10730	6	10	NULL	0	NULL	RXRbeta	NULL		is a type of	NULL				retinoid receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_8_4355_s_161	8626785	A limitation of these experiments was that  HeLa cells contain multiple retinoid receptors (RARalpha, RAR ,  RXRbeta),   and the ligand used in these studies (ATRA) can  activate both classes of receptors (it binds to RARs directly and can  be isomerized  in vivo  to 9- cis-RA, which binds to  RXRs).	bind
47666	1	10732	5	13	NULL	NULL	NULL	Grb	GP		bind					dynamin	GP		proline-rich tail		NULL	in vivo	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1538_1_10_s_184	11341978	A limited number of these in vitro interactions occur in vivo, including binding of Grb2, amphiphysin, PLC  and src to dynamin's proline-rich tail and binding of    subunits of heterotrimeric G proteins to the PH domain.	bind
47667	2	10732	5	13	NULL	NULL	NULL	amphiphysin	GP		bind					dynamin	GP		proline-rich tail		NULL	in vivo	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1538_1_10_s_184	11341978	A limited number of these in vitro interactions occur in vivo, including binding of Grb2, amphiphysin, PLC  and src to dynamin's proline-rich tail and binding of    subunits of heterotrimeric G proteins to the PH domain.	bind
47668	3	10732	5	13	NULL	NULL	NULL	PLC 	GP		bind					dynamin	GP		proline-rich tail		NULL	in vivo	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1538_1_10_s_184	11341978	A limited number of these in vitro interactions occur in vivo, including binding of Grb2, amphiphysin, PLC  and src to dynamin's proline-rich tail and binding of    subunits of heterotrimeric G proteins to the PH domain.	bind
47669	4	10732	5	13	NULL	NULL	NULL	src	GP		bind					dynamin	GP		proline-rich tail		NULL	in vivo	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1538_1_10_s_184	11341978	A limited number of these in vitro interactions occur in vivo, including binding of Grb2, amphiphysin, PLC  and src to dynamin's proline-rich tail and binding of    subunits of heterotrimeric G proteins to the PH domain.	bind
47670	5	10732	5	13	NULL	NULL	NULL	 G protein	GP		bind			heterotrimeric					PH domain		NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1538_1_10_s_184	11341978	A limited number of these in vitro interactions occur in vivo, including binding of Grb2, amphiphysin, PLC  and src to dynamin's proline-rich tail and binding of    subunits of heterotrimeric G proteins to the PH domain.	bind
46992	1	10732	6	NULL	NULL	0	NULL	Grb2	NULL		bind	NULL				dynamin	NULL		proline-rich tail		NULL	in vivo	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1538_1_10_s_184	11341978	A limited number of these in vitro interactions occur in vivo, including binding of Grb2, amphiphysin, PLC  and src to dynamin's proline-rich tail and binding of    subunits of heterotrimeric G proteins to the PH domain.	bind
46993	2	10732	6	NULL	NULL	0	NULL	amphiphysin	NULL		bind	NULL				dynamin	NULL		proline-rich tail		NULL	in vivo	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1538_1_10_s_184	11341978	A limited number of these in vitro interactions occur in vivo, including binding of Grb2, amphiphysin, PLC  and src to dynamin's proline-rich tail and binding of    subunits of heterotrimeric G proteins to the PH domain.	bind
46994	3	10732	6	NULL	NULL	0	NULL	PLC	NULL		bind	NULL				dynamin	NULL		proline-rich tail		NULL	in vivo	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1538_1_10_s_184	11341978	A limited number of these in vitro interactions occur in vivo, including binding of Grb2, amphiphysin, PLC  and src to dynamin's proline-rich tail and binding of    subunits of heterotrimeric G proteins to the PH domain.	bind
46995	4	10732	6	NULL	NULL	0	NULL	src	NULL		bind	NULL				dynamin	NULL		proline-rich tail		NULL	in vivo	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1538_1_10_s_184	11341978	A limited number of these in vitro interactions occur in vivo, including binding of Grb2, amphiphysin, PLC  and src to dynamin's proline-rich tail and binding of    subunits of heterotrimeric G proteins to the PH domain.	bind
46996	5	10732	6	10	NULL	0	NULL	G protein subunit	NULL		bind	NULL		heterotrimeric			NULL		PH domain		NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1538_1_10_s_184	11341978	A limited number of these in vitro interactions occur in vivo, including binding of Grb2, amphiphysin, PLC  and src to dynamin's proline-rich tail and binding of    subunits of heterotrimeric G proteins to the PH domain.	bind
47671	1	10733	5	13	NULL	NULL	NULL				bind			SH2 domains		BCR	GP				NULL		NULL	NULL	NULL	NULL	gw60_structure_3_10_1075_s_379	8590002	A limited set of SH2 domains binds BCR through a high-affinity phosphotyrosine-independent interactions.	bind
47672	2	10733	5	13	NULL	NULL	NULL	statement 1	Process		is independent of					phosphotyrosine	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_structure_3_10_1075_s_379	8590002	A limited set of SH2 domains binds BCR through a high-affinity phosphotyrosine-independent interactions.	bind
46997	1	10733	6	NULL	NULL	0	NULL		NULL		bind	NULL		SH2 domain		BCR	NULL				NULL		0	NULL	NULL	NULL	gw60_structure_3_10_1075_s_379	8590002	A limited set of SH2 domains binds BCR through a high-affinity phosphotyrosine-independent interactions.	bind
46998	2	10733	6	NULL	NULL	0	NULL	statement 1	NULL		is independent of	NULL				phosphotyrosine	NULL				NULL		0	NULL	NULL	NULL	gw60_structure_3_10_1075_s_379	8590002	A limited set of SH2 domains binds BCR through a high-affinity phosphotyrosine-independent interactions.	bind
47673	1	10734	5	13	NULL	NULL	NULL	pol I	GP		bind		low efficiency			Rrn3p	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_pnas_98_25_14334_s_242	11717393	A limiting amount of properly phosphorylated pol I would also explain why the  in vitro binding efficiency of pol I and Rrn3p was rather low although the interaction was strikingly stable.	bind
47003	1	10734	6	NULL	NULL	0	NULL	pol I	NULL		bind	NULL	low efficiency			Rrn3p	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_pnas_98_25_14334_s_242	11717393	A limiting amount of properly phosphorylated pol I would also explain why the  in vitro binding efficiency of pol I and Rrn3p was rather low although the interaction was strikingly stable.	bind
47674	1	10735	5	13	NULL	NULL	NULL	MyD88	GP		is a type of					adapter protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_19_17210_s_13	12618429	A linear activation sequence following engagement of the type I IL-1 receptor (IL-1RI) has been intensely studied and involves binding of the MyD88 and Tollip adapters to the IL-1 receptor chains ( ,  ) with subsequent recruitment of IL-1 receptor-associated kinase ( ,  ).	bind
47675	2	10735	5	13	NULL	NULL	NULL	Tollip	GP		is a type of					adapter protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_19_17210_s_13	12618429	A linear activation sequence following engagement of the type I IL-1 receptor (IL-1RI) has been intensely studied and involves binding of the MyD88 and Tollip adapters to the IL-1 receptor chains ( ,  ) with subsequent recruitment of IL-1 receptor-associated kinase ( ,  ).	bind
47676	3	10735	5	13	NULL	NULL	NULL	MyD88	GP		bind					IL-1 receptor chains	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_19_17210_s_13	12618429	A linear activation sequence following engagement of the type I IL-1 receptor (IL-1RI) has been intensely studied and involves binding of the MyD88 and Tollip adapters to the IL-1 receptor chains ( ,  ) with subsequent recruitment of IL-1 receptor-associated kinase ( ,  ).	bind
47677	4	10735	5	13	NULL	NULL	NULL	Tollip	GP		bind					IL-1 receptor chains	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_19_17210_s_13	12618429	A linear activation sequence following engagement of the type I IL-1 receptor (IL-1RI) has been intensely studied and involves binding of the MyD88 and Tollip adapters to the IL-1 receptor chains ( ,  ) with subsequent recruitment of IL-1 receptor-associated kinase ( ,  ).	bind
47678	5	10735	5	13	NULL	NULL	NULL	statement 3	Process		leads to					IL-1 receptor-associated kinase	GP	recruitment of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_19_17210_s_13	12618429	A linear activation sequence following engagement of the type I IL-1 receptor (IL-1RI) has been intensely studied and involves binding of the MyD88 and Tollip adapters to the IL-1 receptor chains ( ,  ) with subsequent recruitment of IL-1 receptor-associated kinase ( ,  ).	bind
47679	6	10735	5	13	NULL	NULL	NULL	statement 4	Process		leads to					IL-1 receptor-associated kinase	GP	recruitment of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_19_17210_s_13	12618429	A linear activation sequence following engagement of the type I IL-1 receptor (IL-1RI) has been intensely studied and involves binding of the MyD88 and Tollip adapters to the IL-1 receptor chains ( ,  ) with subsequent recruitment of IL-1 receptor-associated kinase ( ,  ).	bind
50352	7	10735	5	13	NULL	NULL	NULL	IL-1RI	GP		is					type I IL-1 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_19_17210_s_13	12618429	A linear activation sequence following engagement of the type I IL-1 receptor (IL-1RI) has been intensely studied and involves binding of the MyD88 and Tollip adapters to the IL-1 receptor chains ( ,  ) with subsequent recruitment of IL-1 receptor-associated kinase ( ,  ).	bind
47004	1	10735	6	NULL	NULL	0	NULL	MyD88	NULL		bind	NULL				IL-1 receptor chains	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_19_17210_s_13	12618429	A linear activation sequence following engagement of the type I IL-1 receptor (IL-1RI) has been intensely studied and involves binding of the MyD88 and Tollip adapters to the IL-1 receptor chains ( ,  ) with subsequent recruitment of IL-1 receptor-associated kinase ( ,  ).	bind
47005	2	10735	6	NULL	NULL	0	NULL	Tollip	NULL		bind	NULL				IL-1 receptor chains	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_19_17210_s_13	12618429	A linear activation sequence following engagement of the type I IL-1 receptor (IL-1RI) has been intensely studied and involves binding of the MyD88 and Tollip adapters to the IL-1 receptor chains ( ,  ) with subsequent recruitment of IL-1 receptor-associated kinase ( ,  ).	bind
47006	3	10735	6	NULL	NULL	0	NULL	Tollip	NULL		is a type of	NULL				adaptor	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_19_17210_s_13	12618429	A linear activation sequence following engagement of the type I IL-1 receptor (IL-1RI) has been intensely studied and involves binding of the MyD88 and Tollip adapters to the IL-1 receptor chains ( ,  ) with subsequent recruitment of IL-1 receptor-associated kinase ( ,  ).	bind
47007	4	10735	6	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				IL-1 receptor-associated kinase	NULL	recruitment of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_19_17210_s_13	12618429	A linear activation sequence following engagement of the type I IL-1 receptor (IL-1RI) has been intensely studied and involves binding of the MyD88 and Tollip adapters to the IL-1 receptor chains ( ,  ) with subsequent recruitment of IL-1 receptor-associated kinase ( ,  ).	bind
47009	5	10735	6	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				IL-1 receptor-associated kinase	NULL	recruitment of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_19_17210_s_13	12618429	A linear activation sequence following engagement of the type I IL-1 receptor (IL-1RI) has been intensely studied and involves binding of the MyD88 and Tollip adapters to the IL-1 receptor chains ( ,  ) with subsequent recruitment of IL-1 receptor-associated kinase ( ,  ).	bind
50353	6	10735	6	10	NULL	0	NULL	MyD88	NULL		is a type of	NULL				adapter	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_19_17210_s_13	12618429	A linear activation sequence following engagement of the type I IL-1 receptor (IL-1RI) has been intensely studied and involves binding of the MyD88 and Tollip adapters to the IL-1 receptor chains ( ,  ) with subsequent recruitment of IL-1 receptor-associated kinase ( ,  ).	bind
50354	7	10735	6	10	NULL	0	NULL	IL-1RI	NULL		is 	NULL				 type I IL-1 receptor	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_19_17210_s_13	12618429	A linear activation sequence following engagement of the type I IL-1 receptor (IL-1RI) has been intensely studied and involves binding of the MyD88 and Tollip adapters to the IL-1 receptor chains ( ,  ) with subsequent recruitment of IL-1 receptor-associated kinase ( ,  ).	bind
47681	1	10738	5	13	NULL	NULL	NULL	PDTI	GP		bind					trypsin	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1621_2_170_s_193	12726993	A linear extrapolation to obtain 100% inhibition indicated that PDTI bound both  trypsins in a 1:1 molar ratio ( Fig. 2), whereas there was no obvious stoichiometry with chymotrypsin.	bind
47013	1	10738	6	NULL	NULL	0	NULL	PDTI	NULL		bind	NULL				trypsin	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1621_2_170_s_193	12726993	A linear extrapolation to obtain 100% inhibition indicated that PDTI bound both  trypsins in a 1:1 molar ratio ( Fig. 2), whereas there was no obvious stoichiometry with chymotrypsin.	bind
47682	1	10739	5	13	NULL	NULL	NULL	actin	GP		bind					mX-S1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_15_15071_s_300	15705568	A linear fit to the same data set (not shown) yielded an apparent second-order  rate constant of actin binding to the mX-S1.	bind
47015	1	10739	6	NULL	NULL	0	NULL	actin	NULL		bind	NULL				mX-S1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_15_15071_s_300	15705568	A linear fit to the same data set (not shown) yielded an apparent second-order  rate constant of actin binding to the mX-S1.	bind
47683	1	10740	5	13	NULL	NULL	NULL	MC-2 	GP		is derived from					IFN	GP		heparin-binding region		NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_74_0_385_s_322	15952892	A linear octapeptide,  MC-2, derived from the heparin-binding region of IFN , significantly prolonged skin  graft survival in an experimental rat model of skin transplantation when it was administered  directly into the graft via osmotic mini pumps ( 83).	bind
47684	2	10740	5	13	NULL	NULL	NULL	statement 1	Process		prolonged		significantly			skin graft	OrganismPart	survival of			NULL	experimental rat model	NULL	NULL	NULL	NULL	gw70_annurevbiochem_74_0_385_s_322	15952892	A linear octapeptide,  MC-2, derived from the heparin-binding region of IFN , significantly prolonged skin  graft survival in an experimental rat model of skin transplantation when it was administered  directly into the graft via osmotic mini pumps ( 83).	bind
50355	3	10740	5	13	NULL	NULL	NULL	MC-2	GP		is a type of					linear octapeptide	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_74_0_385_s_322	15952892	A linear octapeptide,  MC-2, derived from the heparin-binding region of IFN , significantly prolonged skin  graft survival in an experimental rat model of skin transplantation when it was administered  directly into the graft via osmotic mini pumps ( 83).	bind
47016	1	10740	6	NULL	NULL	0	NULL	MC-2	NULL		is a type of	NULL				linear octapeptide	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_74_0_385_s_322	15952892	A linear octapeptide,  MC-2, derived from the heparin-binding region of IFN , significantly prolonged skin  graft survival in an experimental rat model of skin transplantation when it was administered  directly into the graft via osmotic mini pumps ( 83).	bind
47017	2	10740	6	NULL	NULL	0	NULL	MC-2	NULL		is derived from	NULL				IFN	NULL		heparin-binding region		NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_74_0_385_s_322	15952892	A linear octapeptide,  MC-2, derived from the heparin-binding region of IFN , significantly prolonged skin  graft survival in an experimental rat model of skin transplantation when it was administered  directly into the graft via osmotic mini pumps ( 83).	bind
47020	3	10740	6	NULL	NULL	0	NULL	MC-2	NULL		prolonged	NULL				skin graft survival	NULL				NULL	experimental rat model of skin transplantation	0	NULL	NULL	NULL	gw70_annurevbiochem_74_0_385_s_322	15952892	A linear octapeptide,  MC-2, derived from the heparin-binding region of IFN , significantly prolonged skin  graft survival in an experimental rat model of skin transplantation when it was administered  directly into the graft via osmotic mini pumps ( 83).	bind
47685	1	10745	5	13	NULL	NULL	NULL	Arf	GP		bind					Golgi membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_28_16952_s_188	8663371	A link between Arf and PKC seems to be established by the observation that activation of the latter leads to enhanced binding of Arf and beta-COP to Golgi membranes ( 19).	bind
47686	2	10745	5	13	NULL	NULL	NULL	beta-COP	GP		bind					Golgi membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_28_16952_s_188	8663371	A link between Arf and PKC seems to be established by the observation that activation of the latter leads to enhanced binding of Arf and beta-COP to Golgi membranes ( 19).	bind
47687	3	10745	5	13	NULL	NULL	NULL	PKC	GP	activation of	enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_28_16952_s_188	8663371	A link between Arf and PKC seems to be established by the observation that activation of the latter leads to enhanced binding of Arf and beta-COP to Golgi membranes ( 19).	bind
47688	4	10745	5	13	NULL	NULL	NULL	PKC	GP	activation of	enhances					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_28_16952_s_188	8663371	A link between Arf and PKC seems to be established by the observation that activation of the latter leads to enhanced binding of Arf and beta-COP to Golgi membranes ( 19).	bind
47021	1	10745	6	NULL	NULL	0	NULL	Arf 	NULL		bind	NULL				Golgi membrane	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_28_16952_s_188	8663371	A link between Arf and PKC seems to be established by the observation that activation of the latter leads to enhanced binding of Arf and beta-COP to Golgi membranes ( 19).	bind
47022	2	10745	6	NULL	NULL	0	NULL	beta-COP	NULL		bind	NULL				Golgi membranes	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_28_16952_s_188	8663371	A link between Arf and PKC seems to be established by the observation that activation of the latter leads to enhanced binding of Arf and beta-COP to Golgi membranes ( 19).	bind
47023	3	10745	6	10	NULL	0	NULL	PKC		activation of	enhances					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_28_16952_s_188	8663371	A link between Arf and PKC seems to be established by the observation that activation of the latter leads to enhanced binding of Arf and beta-COP to Golgi membranes ( 19).	bind
47024	4	10745	6	10	NULL	0	NULL	PKC		activation of	enhances					statement 2					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_28_16952_s_188	8663371	A link between Arf and PKC seems to be established by the observation that activation of the latter leads to enhanced binding of Arf and beta-COP to Golgi membranes ( 19).	bind
47736	1	10746	5	13	NULL	NULL	NULL	simian virus 40 large T antigen	GP		bind					p53	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_7_2358_s_264	10713160	A link between p53 and CDF-1 is further supported by the recent observation that simian virus 40 large T antigen, which binds and inactivates p53, prevents CDF-1 from binding to CDE elements in WI-38 cells ( 63).	bind
47737	2	10746	5	13	NULL	NULL	NULL	statement 1	Process		inactivates					p53	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_7_2358_s_264	10713160	A link between p53 and CDF-1 is further supported by the recent observation that simian virus 40 large T antigen, which binds and inactivates p53, prevents CDF-1 from binding to CDE elements in WI-38 cells ( 63).	bind
47738	3	10746	5	13	NULL	NULL	NULL	CDF-1	GP		bind									CDE elements	NULL	WI-38 cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_7_2358_s_264	10713160	A link between p53 and CDF-1 is further supported by the recent observation that simian virus 40 large T antigen, which binds and inactivates p53, prevents CDF-1 from binding to CDE elements in WI-38 cells ( 63).	bind
47739	4	10746	5	13	NULL	NULL	NULL	simian virus 40 large T antigen	GP		prevents					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_7_2358_s_264	10713160	A link between p53 and CDF-1 is further supported by the recent observation that simian virus 40 large T antigen, which binds and inactivates p53, prevents CDF-1 from binding to CDE elements in WI-38 cells ( 63).	bind
47025	1	10746	6	NULL	NULL	0	NULL	simian virus 40 large T antigen	NULL		bind	NULL				p53	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_7_2358_s_264	10713160	A link between p53 and CDF-1 is further supported by the recent observation that simian virus 40 large T antigen, which binds and inactivates p53, prevents CDF-1 from binding to CDE elements in WI-38 cells ( 63).	bind
47026	2	10746	6	NULL	NULL	0	NULL	simian virus 40 large T antigen	NULL		inactivates	NULL				p53	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_7_2358_s_264	10713160	A link between p53 and CDF-1 is further supported by the recent observation that simian virus 40 large T antigen, which binds and inactivates p53, prevents CDF-1 from binding to CDE elements in WI-38 cells ( 63).	bind
47027	3	10746	6	NULL	NULL	0	NULL	CDF-1	NULL		bind	NULL					NULL			CDE element	NULL	WI-38 cells	0	NULL	NULL	NULL	gw60_molcellbiol_20_7_2358_s_264	10713160	A link between p53 and CDF-1 is further supported by the recent observation that simian virus 40 large T antigen, which binds and inactivates p53, prevents CDF-1 from binding to CDE elements in WI-38 cells ( 63).	bind
47031	4	10746	6	NULL	NULL	0	NULL	simian virus 40 large T antigen	NULL		prevents	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_7_2358_s_264	10713160	A link between p53 and CDF-1 is further supported by the recent observation that simian virus 40 large T antigen, which binds and inactivates p53, prevents CDF-1 from binding to CDE elements in WI-38 cells ( 63).	bind
47740	1	10747	5	13	NULL	NULL	NULL	IL-8	GP	native	bind					CXCR1 peptide	GP		N-domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_35_36175_s_117	15252057	A linkage scheme of native IL-8 binding to CXCR1 N-domain peptide.	bind
47034	1	10747	6	NULL	NULL	0	NULL	IL-8	NULL	native	bind	NULL				CXCR1	NULL		N-domain peptide		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_35_36175_s_117	15252057	A linkage scheme of native IL-8 binding to CXCR1 N-domain peptide.	bind
47741	1	10748	5	13	NULL	NULL	NULL				exits between			linker region		Vinexin	GP		second SH3 domain & third SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_13053_s_107	11825889	A Linker Region between the Second and Third SH3 Domains of Vinexin beta Is Necessary for Anchorage-independent ERK2 Activation-- The first and second SH3 domains of vinexin beta bind to vinculin, and the third SH3 domain binds to Sos.	bind
47742	2	10748	5	13	NULL	NULL	NULL	ERK2	GP	activation of	is independent of					anchorage	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_13053_s_107	11825889	A Linker Region between the Second and Third SH3 Domains of Vinexin beta Is Necessary for Anchorage-independent ERK2 Activation-- The first and second SH3 domains of vinexin beta bind to vinculin, and the third SH3 domain binds to Sos.	bind
47743	3	10748	5	13	NULL	NULL	NULL	statement 1	Process		is necessary for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_13053_s_107	11825889	A Linker Region between the Second and Third SH3 Domains of Vinexin beta Is Necessary for Anchorage-independent ERK2 Activation-- The first and second SH3 domains of vinexin beta bind to vinculin, and the third SH3 domain binds to Sos.	bind
47744	4	10748	5	13	NULL	NULL	NULL	vinexin beta	GP		bind			SH3 domain		vinculin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_13053_s_107	11825889	A Linker Region between the Second and Third SH3 Domains of Vinexin beta Is Necessary for Anchorage-independent ERK2 Activation-- The first and second SH3 domains of vinexin beta bind to vinculin, and the third SH3 domain binds to Sos.	bind
47745	5	10748	5	13	NULL	NULL	NULL	vinexin beta	GP		bind			SH3 domain		Sos	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_13053_s_107	11825889	A Linker Region between the Second and Third SH3 Domains of Vinexin beta Is Necessary for Anchorage-independent ERK2 Activation-- The first and second SH3 domains of vinexin beta bind to vinculin, and the third SH3 domain binds to Sos.	bind
47035	1	10748	6	NULL	NULL	0	NULL	vinexin beta	NULL		bind	NULL		first and second SH3 domain		vinculin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_13053_s_107	11825889	A Linker Region between the Second and Third SH3 Domains of Vinexin beta Is Necessary for Anchorage-independent ERK2 Activation-- The first and second SH3 domains of vinexin beta bind to vinculin, and the third SH3 domain binds to Sos.	bind
47036	2	10748	6	NULL	NULL	0	NULL	vinexin beta	NULL		bind	NULL		third SH3 domain		Sos	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_13053_s_107	11825889	A Linker Region between the Second and Third SH3 Domains of Vinexin beta Is Necessary for Anchorage-independent ERK2 Activation-- The first and second SH3 domains of vinexin beta bind to vinculin, and the third SH3 domain binds to Sos.	bind
47037	5	10748	6	10	NULL	0	NULL	statement 4	NULL		is necessary for	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_13053_s_107	11825889	A Linker Region between the Second and Third SH3 Domains of Vinexin beta Is Necessary for Anchorage-independent ERK2 Activation-- The first and second SH3 domains of vinexin beta bind to vinculin, and the third SH3 domain binds to Sos.	bind
47038	3	10748	6	NULL	NULL	0	NULL	ERK2	NULL	activation of	is independent of	NULL				anchorage	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_13053_s_107	11825889	A Linker Region between the Second and Third SH3 Domains of Vinexin beta Is Necessary for Anchorage-independent ERK2 Activation-- The first and second SH3 domains of vinexin beta bind to vinculin, and the third SH3 domain binds to Sos.	bind
50356	4	10748	6	10	NULL	0	NULL	linker region	NULL		exist between	NULL				Vinexin beta	NULL		Second and Third SH3 Domains		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_13053_s_107	11825889	A Linker Region between the Second and Third SH3 Domains of Vinexin beta Is Necessary for Anchorage-independent ERK2 Activation-- The first and second SH3 domains of vinexin beta bind to vinculin, and the third SH3 domain binds to Sos.	bind
47746	1	10749	5	13	NULL	NULL	NULL	Leu3p	GP		is a type of					Zinc Cluster Protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_24_15521_s_258	9182587	A Linker Region of the Yeast Zinc Cluster Protein Leu3p Specifies Binding to Everted Repeat DNA.	bind
47747	2	10749	5	13	NULL	NULL	NULL	Leu3p	GP	yeast	bind			linker region		everted repeat DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_24_15521_s_258	9182587	A Linker Region of the Yeast Zinc Cluster Protein Leu3p Specifies Binding to Everted Repeat DNA.	bind
47039	1	10749	6	10	NULL	0	NULL	Leu3p		yeast	bind			linker region		Everted Repeat DNA					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_24_15521_s_258	9182587	A Linker Region of the Yeast Zinc Cluster Protein Leu3p Specifies Binding to Everted Repeat DNA.	bind
47040	2	10749	6	NULL	NULL	0	NULL	Leu3p	NULL		is a type of	NULL				Zinc cluster protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_24_15521_s_258	9182587	A Linker Region of the Yeast Zinc Cluster Protein Leu3p Specifies Binding to Everted Repeat DNA.	bind
47748	1	10750	5	13	NULL	NULL	NULL	familial dysbetalipoproteinemia	MedicalFinding		is a type of					lipid disorder	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_10_1719_s_181	7583549	A lipid disorder (familial dysbetalipoproteinemia) affecting apoE, the other ligand known to bind to the LDLR, results in a markedly reduced binding of apoE-containing VLDL remnants to the LDLR.	bind
47749	2	10750	5	13	NULL	NULL	NULL	apoE	GP		is a type of					ligand	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_10_1719_s_181	7583549	A lipid disorder (familial dysbetalipoproteinemia) affecting apoE, the other ligand known to bind to the LDLR, results in a markedly reduced binding of apoE-containing VLDL remnants to the LDLR.	bind
47750	3	10750	5	13	NULL	NULL	NULL	apoE	GP		bind					LDLR	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_10_1719_s_181	7583549	A lipid disorder (familial dysbetalipoproteinemia) affecting apoE, the other ligand known to bind to the LDLR, results in a markedly reduced binding of apoE-containing VLDL remnants to the LDLR.	bind
47751	4	10750	5	13	NULL	NULL	NULL	VLDL remnants	GP	apoE-containing	bind					LDLR	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_10_1719_s_181	7583549	A lipid disorder (familial dysbetalipoproteinemia) affecting apoE, the other ligand known to bind to the LDLR, results in a markedly reduced binding of apoE-containing VLDL remnants to the LDLR.	bind
47752	5	10750	5	13	NULL	NULL	NULL	familial dysbetalipoproteinemia	MedicalFinding		reduces		markedly			statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_10_1719_s_181	7583549	A lipid disorder (familial dysbetalipoproteinemia) affecting apoE, the other ligand known to bind to the LDLR, results in a markedly reduced binding of apoE-containing VLDL remnants to the LDLR.	bind
47041	1	10750	6	NULL	NULL	0	NULL	apoE	NULL		bind	NULL				LDLR	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_10_1719_s_181	7583549	A lipid disorder (familial dysbetalipoproteinemia) affecting apoE, the other ligand known to bind to the LDLR, results in a markedly reduced binding of apoE-containing VLDL remnants to the LDLR.	bind
47042	2	10750	6	NULL	NULL	0	NULL	familial dysbetalipoproteinemia	NULL		is a type of	NULL				lipid disorder	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_10_1719_s_181	7583549	A lipid disorder (familial dysbetalipoproteinemia) affecting apoE, the other ligand known to bind to the LDLR, results in a markedly reduced binding of apoE-containing VLDL remnants to the LDLR.	bind
47043	3	10750	6	NULL	NULL	0	NULL	VLDL remnants	NULL	apoE-containing	bind	NULL				LDLR	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_10_1719_s_181	7583549	A lipid disorder (familial dysbetalipoproteinemia) affecting apoE, the other ligand known to bind to the LDLR, results in a markedly reduced binding of apoE-containing VLDL remnants to the LDLR.	bind
47044	4	10750	6	10	NULL	0	NULL	familial dysbetalipoproteinemia			reduces					statement 3					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_10_1719_s_181	7583549	A lipid disorder (familial dysbetalipoproteinemia) affecting apoE, the other ligand known to bind to the LDLR, results in a markedly reduced binding of apoE-containing VLDL remnants to the LDLR.	bind
50357	5	10750	6	10	NULL	0	NULL	apoE	NULL		is a type of	NULL				ligand	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_10_1719_s_181	7583549	A lipid disorder (familial dysbetalipoproteinemia) affecting apoE, the other ligand known to bind to the LDLR, results in a markedly reduced binding of apoE-containing VLDL remnants to the LDLR.	bind
47753	1	10751	5	13	NULL	NULL	NULL	LmB	GP		is a type of					lipoprotein	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2408_s_27	11953377	A lipoprotein, designated LmB, which binds to both Fn and laminin was cloned from GBS, but it was not shown to be involved in adherence or invasion of epithelial cells ( 23).	bind
47754	2	10751	5	13	NULL	NULL	NULL	LmB	GP		bind					Fn	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2408_s_27	11953377	A lipoprotein, designated LmB, which binds to both Fn and laminin was cloned from GBS, but it was not shown to be involved in adherence or invasion of epithelial cells ( 23).	bind
47755	3	10751	5	13	NULL	NULL	NULL	LmB	GP		bind					laminin	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2408_s_27	11953377	A lipoprotein, designated LmB, which binds to both Fn and laminin was cloned from GBS, but it was not shown to be involved in adherence or invasion of epithelial cells ( 23).	bind
47756	4	10751	5	13	NULL	NULL	NULL	LmB	GP		is not involved in					epithelial cells	Cell	adherence of			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2408_s_27	11953377	A lipoprotein, designated LmB, which binds to both Fn and laminin was cloned from GBS, but it was not shown to be involved in adherence or invasion of epithelial cells ( 23).	bind
47757	5	10751	5	13	NULL	NULL	NULL	LmB	GP		is not involved in					epithelial cells	Cell	invasion of			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2408_s_27	11953377	A lipoprotein, designated LmB, which binds to both Fn and laminin was cloned from GBS, but it was not shown to be involved in adherence or invasion of epithelial cells ( 23).	bind
47045	1	10751	6	NULL	NULL	0	NULL	LmB	NULL		is a type of	NULL				lipoprotein	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_5_2408_s_27	11953377	A lipoprotein, designated LmB, which binds to both Fn and laminin was cloned from GBS, but it was not shown to be involved in adherence or invasion of epithelial cells ( 23).	bind
47046	2	10751	6	NULL	NULL	0	NULL	LmB	NULL		bind	NULL				Fn	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_5_2408_s_27	11953377	A lipoprotein, designated LmB, which binds to both Fn and laminin was cloned from GBS, but it was not shown to be involved in adherence or invasion of epithelial cells ( 23).	bind
47047	3	10751	6	NULL	NULL	0	NULL	LmB	NULL		bind	NULL				laminin	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_70_5_2408_s_27	11953377	A lipoprotein, designated LmB, which binds to both Fn and laminin was cloned from GBS, but it was not shown to be involved in adherence or invasion of epithelial cells ( 23).	bind
47048	4	10751	6	10	NULL	0	NULL	LmB	NULL		is not involved in	NULL				epithelial cells	NULL	adherence of 			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2408_s_27	11953377	A lipoprotein, designated LmB, which binds to both Fn and laminin was cloned from GBS, but it was not shown to be involved in adherence or invasion of epithelial cells ( 23).	bind
47049	5	10751	6	10	NULL	0	NULL	LmB	NULL		is not involved in	NULL				epithelial cells	NULL	invasion of 			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_5_2408_s_27	11953377	A lipoprotein, designated LmB, which binds to both Fn and laminin was cloned from GBS, but it was not shown to be involved in adherence or invasion of epithelial cells ( 23).	bind
50761	1	10752	5	13	NULL	NULL	NULL	fibulin-2 	GP		bind					gamma2-r	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_5_2814_s_55	9006922	A list of synthetic peptides from the N-terminus of domain IV of the gamma2 chain and their activities for competing fibulin-2 binding to gamma2-r    he activities shown were from the competition assays in Fig 4. ++, active at 200 mug/ml; +, active at 1 mg/ml;  , inactive even at 1 mg/ml.	bind
50814	1	10752	6	NULL	NULL	0	NULL	fibulin-2	NULL		bind	NULL				gamma2-r	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_5_2814_s_55	9006922	A list of synthetic peptides from the N-terminus of domain IV of the gamma2 chain and their activities for competing fibulin-2 binding to gamma2-r    he activities shown were from the competition assays in Fig 4. ++, active at 200 mug/ml; +, active at 1 mg/ml;  , inactive even at 1 mg/ml.	bind
47759	1	10753	5	13	NULL	NULL	NULL	calmodulin	GP		bind					IQGAP1	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_542_1_7_s_89	12729888	A localized increase in [Ca2+]i increases the binding of calmodulin to IQGAP1.	bind
47760	2	10753	5	13	NULL	NULL	NULL	Ca2+	Chemical	increase in	increases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_542_1_7_s_89	12729888	A localized increase in [Ca2+]i increases the binding of calmodulin to IQGAP1.	bind
47050	1	10753	6	NULL	NULL	0	NULL	calmodulin	NULL		bind	NULL				IQGAP1	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_542_1_7_s_89	12729888	A localized increase in [Ca2+]i increases the binding of calmodulin to IQGAP1.	bind
47051	2	10753	6	NULL	NULL	0	NULL	[Ca2+]	NULL	increase in	increases	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_542_1_7_s_89	12729888	A localized increase in [Ca2+]i increases the binding of calmodulin to IQGAP1.	bind
47761	1	10754	5	13	NULL	NULL	NULL	TFIID subunit	GP		bind					TBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_23_17391_s_127	10751405	A logical explanation for these findings is that in the absence of TAFII145p another TFIID subunit binds to TBP and protects it from degradation.	bind
47762	2	10754	5	13	NULL	NULL	NULL	statement 1	Process		protects					TBP	GP	degradation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_23_17391_s_127	10751405	A logical explanation for these findings is that in the absence of TAFII145p another TFIID subunit binds to TBP and protects it from degradation.	bind
47763	3	10754	5	13	NULL	NULL	NULL	statement 1	Process		in the absence of					TAFII145p	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_23_17391_s_127	10751405	A logical explanation for these findings is that in the absence of TAFII145p another TFIID subunit binds to TBP and protects it from degradation.	bind
47052	1	10754	6	NULL	NULL	0	NULL	TFIID subunit	NULL		bind	NULL				TBP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_23_17391_s_127	10751405	A logical explanation for these findings is that in the absence of TAFII145p another TFIID subunit binds to TBP and protects it from degradation.	bind
47053	2	10754	6	NULL	NULL	0	NULL	statement 1	NULL		occurs in absence of	NULL				TAFII145p	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_23_17391_s_127	10751405	A logical explanation for these findings is that in the absence of TAFII145p another TFIID subunit binds to TBP and protects it from degradation.	bind
47054	3	10754	6	NULL	NULL	0	NULL	statement 1	NULL		protects	NULL				TBP	NULL	degradation of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_23_17391_s_127	10751405	A logical explanation for these findings is that in the absence of TAFII145p another TFIID subunit binds to TBP and protects it from degradation.	bind
47764	1	10755	5	13	NULL	NULL	NULL	TFIID subunits	GP		bind					TBP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_23_17391_s_27	10751405	A logical explanation for these observations is that additional TFIID subunits bind to TBP in the absence of TAFII145p, and that the histone-like TAFIIs are more important for TFIID structure.	bind
47765	2	10755	5	13	NULL	NULL	NULL	statement 1	Process		in the absence of					TAFII145p	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_23_17391_s_27	10751405	A logical explanation for these observations is that additional TFIID subunits bind to TBP in the absence of TAFII145p, and that the histone-like TAFIIs are more important for TFIID structure.	bind
47766	3	10755	5	13	NULL	NULL	NULL	 TAFIIs	GP	histone-like	is important for					TFIID 	GP	structure of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_23_17391_s_27	10751405	A logical explanation for these observations is that additional TFIID subunits bind to TBP in the absence of TAFII145p, and that the histone-like TAFIIs are more important for TFIID structure.	bind
47055	1	10755	6	NULL	NULL	0	NULL	TFIID subunit	NULL		bind	NULL				TBP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_23_17391_s_27	10751405	A logical explanation for these observations is that additional TFIID subunits bind to TBP in the absence of TAFII145p, and that the histone-like TAFIIs are more important for TFIID structure.	bind
47056	2	10755	6	NULL	NULL	0	NULL	statement 1	NULL		occurs in absence of	NULL				TAFII145p	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_23_17391_s_27	10751405	A logical explanation for these observations is that additional TFIID subunits bind to TBP in the absence of TAFII145p, and that the histone-like TAFIIs are more important for TFIID structure.	bind
47057	3	10755	6	NULL	NULL	0	NULL	TAFIIs	NULL	histone-like	are important for	NULL				TFIID	NULL	structure of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_23_17391_s_27	10751405	A logical explanation for these observations is that additional TFIID subunits bind to TBP in the absence of TAFII145p, and that the histone-like TAFIIs are more important for TFIID structure.	bind
47767	1	10756	5	13	NULL	NULL	NULL	L1	GP		bind					PDP1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_14976_s_331	11842080	A logical explanation is that the native Ser-Leu residues of L1 do not allow the corresponding Glu55 side chain to be properly positioned for abetting binding of L1 to PDP1.	bind
47768	2	10756	5	13	NULL	NULL	NULL	L1	GP	native	does not allow			Ser-Leu residues				proper positioning of	Glu55 side chain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_14976_s_331	11842080	A logical explanation is that the native Ser-Leu residues of L1 do not allow the corresponding Glu55 side chain to be properly positioned for abetting binding of L1 to PDP1.	bind
47769	3	10756	5	13	NULL	NULL	NULL			\t	abet			Glu55 side chain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_14976_s_331	11842080	A logical explanation is that the native Ser-Leu residues of L1 do not allow the corresponding Glu55 side chain to be properly positioned for abetting binding of L1 to PDP1.	bind
47058	1	10756	6	NULL	NULL	0	NULL	L1	NULL		bind	NULL				PDP1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_17_14976_s_331	11842080	A logical explanation is that the native Ser-Leu residues of L1 do not allow the corresponding Glu55 side chain to be properly positioned for abetting binding of L1 to PDP1.	bind
47059	2	10756	6	NULL	NULL	0	NULL	L1	NULL	native	do not allow	NULL		Ser-Leu residue			NULL	positioning of	Glu55 side chain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_17_14976_s_331	11842080	A logical explanation is that the native Ser-Leu residues of L1 do not allow the corresponding Glu55 side chain to be properly positioned for abetting binding of L1 to PDP1.	bind
47060	3	10756	6	NULL	NULL	0	NULL		NULL		abett	NULL		Glu55 side chain		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_17_14976_s_331	11842080	A logical explanation is that the native Ser-Leu residues of L1 do not allow the corresponding Glu55 side chain to be properly positioned for abetting binding of L1 to PDP1.	bind
47770	1	10757	5	13	NULL	NULL	NULL	transcription factor	GP		bind							p53-regulated		promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_10_8261_s_256	12475992	A logical extension of these observations is that there may be a transcription factor that binds to p53-regulated promoters and establishes the open chromatin confirmation prior to p53 activation.	bind
47771	2	10757	5	13	NULL	NULL	NULL	statement 1	Process		establishes					open chromatin confirmation	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_10_8261_s_256	12475992	A logical extension of these observations is that there may be a transcription factor that binds to p53-regulated promoters and establishes the open chromatin confirmation prior to p53 activation.	bind
47772	3	10757	5	13	NULL	NULL	NULL	statement 2	Process		occurs prior to					p53	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_10_8261_s_256	12475992	A logical extension of these observations is that there may be a transcription factor that binds to p53-regulated promoters and establishes the open chromatin confirmation prior to p53 activation.	bind
47062	1	10757	6	NULL	NULL	0	NULL	transcription factor	NULL		bind	NULL					NULL	p53-regulated		promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_10_8261_s_256	12475992	A logical extension of these observations is that there may be a transcription factor that binds to p53-regulated promoters and establishes the open chromatin confirmation prior to p53 activation.	bind
47063	2	10757	6	10	NULL	0	NULL	statement 1	NULL		establishes	NULL				open chromatin confirmation	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_10_8261_s_256	12475992	A logical extension of these observations is that there may be a transcription factor that binds to p53-regulated promoters and establishes the open chromatin confirmation prior to p53 activation.	bind
47064	3	10757	6	NULL	NULL	0	NULL	statement 2	NULL		occurs before	NULL				p53	NULL	activation of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_10_8261_s_256	12475992	A logical extension of these observations is that there may be a transcription factor that binds to p53-regulated promoters and establishes the open chromatin confirmation prior to p53 activation.	bind
47773	1	10758	5	13	NULL	NULL	NULL	GroES	GP		bind					Gp31	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_34_0_439_s_175	11092834	A logical extrapolation of the results detailed above would be that the GroEL(E191G)  mutant protein spends more time in the closed state, thus disfavoring GroES and Gp31  binding.	bind
47774	2	10758	5	13	NULL	NULL	NULL	GroEL	GP	mutant	is present in			E191G		closed state					NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_34_0_439_s_175	11092834	A logical extrapolation of the results detailed above would be that the GroEL(E191G)  mutant protein spends more time in the closed state, thus disfavoring GroES and Gp31  binding.	bind
47775	3	10758	5	13	NULL	NULL	NULL	statement 2	Process		disfavor					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_34_0_439_s_175	11092834	A logical extrapolation of the results detailed above would be that the GroEL(E191G)  mutant protein spends more time in the closed state, thus disfavoring GroES and Gp31  binding.	bind
47065	1	10758	6	NULL	NULL	0	NULL	GroES	NULL		bind	NULL				Gp31	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevgenet_34_0_439_s_175	11092834	A logical extrapolation of the results detailed above would be that the GroEL(E191G)  mutant protein spends more time in the closed state, thus disfavoring GroES and Gp31  binding.	bind
47066	2	10758	6	NULL	NULL	0	NULL	GroEL protein	NULL	mutant	is in 	NULL		E191G		closed confirmation	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevgenet_34_0_439_s_175	11092834	A logical extrapolation of the results detailed above would be that the GroEL(E191G)  mutant protein spends more time in the closed state, thus disfavoring GroES and Gp31  binding.	bind
47067	3	10758	6	NULL	NULL	0	NULL	statement 2	NULL		disfavors	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevgenet_34_0_439_s_175	11092834	A logical extrapolation of the results detailed above would be that the GroEL(E191G)  mutant protein spends more time in the closed state, thus disfavoring GroES and Gp31  binding.	bind
47776	1	10759	5	13	NULL	NULL	NULL	p85	GP		bind		weakly	tyrosine 799;;tyrosine 1173		CKR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_21_17686_s_159	11278468	A long exposure of the blot showed trace evidence of p85 in CKR/F799 and CKR/F1173 but not in CKR/F2 (data not shown), suggesting that binding of p85 to CKR is not strong and both tyrosines 799 and 1173 may be acting as low affinity binding sites for p85.	bind
47273	1	10759	6	10	NULL	0	NULL	p85	NULL		bind	NULL	weakly	tyrosine 799;; tyrosine 1173		CKR	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_21_17686_s_159	11278468	A long exposure of the blot showed trace evidence of p85 in CKR/F799 and CKR/F1173 but not in CKR/F2 (data not shown), suggesting that binding of p85 to CKR is not strong and both tyrosines 799 and 1173 may be acting as low affinity binding sites for p85.	bind
47777	1	10760	5	13	NULL	NULL	NULL	GpIbalpha	GP		bind					thrombin	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_301_5630_222_s_138	12855811	A long O-glycosylated mucin-like stalk (not drawn to scale) of the GpIbalpha receptor places its thrombin binding domain  45 nm away from the platelet membrane surface (  39); thus, platelet membranes that are about 100 nm apart could be linked together by binding interactions between GpIbalpha and thrombin.	bind
47778	2	10760	5	13	NULL	NULL	NULL	platelet membranes	CellComponent		is linked together by					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_301_5630_222_s_138	12855811	A long O-glycosylated mucin-like stalk (not drawn to scale) of the GpIbalpha receptor places its thrombin binding domain  45 nm away from the platelet membrane surface (  39); thus, platelet membranes that are about 100 nm apart could be linked together by binding interactions between GpIbalpha and thrombin.	bind
47779	3	10760	5	13	NULL	NULL	NULL	GpIbalpha receptor	GP		is placed away from			thrombin binding domain		platelet membrane surface	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_science_301_5630_222_s_138	12855811	A long O-glycosylated mucin-like stalk (not drawn to scale) of the GpIbalpha receptor places its thrombin binding domain  45 nm away from the platelet membrane surface (  39); thus, platelet membranes that are about 100 nm apart could be linked together by binding interactions between GpIbalpha and thrombin.	bind
47780	4	10760	5	13	NULL	NULL	NULL	GpIbalpha receptor	GP		is required for			O-glycosylated mucin-like stalk		statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_301_5630_222_s_138	12855811	A long O-glycosylated mucin-like stalk (not drawn to scale) of the GpIbalpha receptor places its thrombin binding domain  45 nm away from the platelet membrane surface (  39); thus, platelet membranes that are about 100 nm apart could be linked together by binding interactions between GpIbalpha and thrombin.	bind
47068	1	10760	6	NULL	NULL	0	NULL	GpIbalpha	NULL		bind	NULL				thrombin	NULL				NULL		0	NULL	NULL	NULL	gw60_science_301_5630_222_s_138	12855811	A long O-glycosylated mucin-like stalk (not drawn to scale) of the GpIbalpha receptor places its thrombin binding domain  45 nm away from the platelet membrane surface (  39); thus, platelet membranes that are about 100 nm apart could be linked together by binding interactions between GpIbalpha and thrombin.	bind
47292	2	10760	6	NULL	NULL	0	NULL	statement 1	NULL		links	NULL				platelet membranes	NULL				NULL		NULL	NULL	NULL	NULL	gw60_science_301_5630_222_s_138	12855811	A long O-glycosylated mucin-like stalk (not drawn to scale) of the GpIbalpha receptor places its thrombin binding domain  45 nm away from the platelet membrane surface (  39); thus, platelet membranes that are about 100 nm apart could be linked together by binding interactions between GpIbalpha and thrombin.	bind
47306	3	10760	6	10	NULL	0	NULL	GpIbalpha receptor			is placed away from			thrombin binding domain		platelet membrane surface					NULL		NULL	NULL	NULL	NULL	gw60_science_301_5630_222_s_138	12855811	A long O-glycosylated mucin-like stalk (not drawn to scale) of the GpIbalpha receptor places its thrombin binding domain  45 nm away from the platelet membrane surface (  39); thus, platelet membranes that are about 100 nm apart could be linked together by binding interactions between GpIbalpha and thrombin.	bind
47308	4	10760	6	10	NULL	0	NULL	GpIbalpha			is required for			long O-glycosylated mucin-like stalk		statement 3					NULL		NULL	NULL	NULL	NULL	gw60_science_301_5630_222_s_138	12855811	A long O-glycosylated mucin-like stalk (not drawn to scale) of the GpIbalpha receptor places its thrombin binding domain  45 nm away from the platelet membrane surface (  39); thus, platelet membranes that are about 100 nm apart could be linked together by binding interactions between GpIbalpha and thrombin.	bind
47781	1	10761	5	13	NULL	NULL	NULL	antibodies	GP	conventional	lacks			VL		antigen-binding surface	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_24774_s_21	11335716	A longer CDR3 increases the antigen-binding surface and partially compensates for the absence of the antigen-binding surface provided by the VL in conventional antibodies ( 3).	bind
47783	2	10761	5	13	NULL	NULL	NULL	CDR3	GP	longer	increases					antigen-binding surface	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_24774_s_21	11335716	A longer CDR3 increases the antigen-binding surface and partially compensates for the absence of the antigen-binding surface provided by the VL in conventional antibodies ( 3).	bind
47784	3	10761	5	13	NULL	NULL	NULL	statement 2	Process		compensates for		partially			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_24774_s_21	11335716	A longer CDR3 increases the antigen-binding surface and partially compensates for the absence of the antigen-binding surface provided by the VL in conventional antibodies ( 3).	bind
47311	1	10761	6	10	NULL	0	NULL	CDR3		longer	increases					antigen-binding surface					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_24774_s_21	11335716	A longer CDR3 increases the antigen-binding surface and partially compensates for the absence of the antigen-binding surface provided by the VL in conventional antibodies ( 3).	bind
47312	2	10761	6	10	NULL	0	NULL	antigen binding surface			is absent in					VL					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_24774_s_21	11335716	A longer CDR3 increases the antigen-binding surface and partially compensates for the absence of the antigen-binding surface provided by the VL in conventional antibodies ( 3).	bind
47315	3	10761	6	NULL	NULL	0	NULL	statement 1	NULL		compensates	NULL	partially			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_27_24774_s_21	11335716	A longer CDR3 increases the antigen-binding surface and partially compensates for the absence of the antigen-binding surface provided by the VL in conventional antibodies ( 3).	bind
47848	1	10762	5	13	NULL	NULL	NULL	Nef	GP		bind					Nef receptor	GP	putative			NULL		NULL	NULL	NULL	NULL	gw60_febslett_422_3_363_s_108	9498817	A longer preincubation period for fasudil hydrochloride was required than for M3, probably because fasudil hydrochloride taken up by cells was converted to an active form M3 during this period [ 10], and thereby impeded transduction of the apoptosis-inducing signal introduced by binding of Nef to a putative Nef receptor, a death-signalling receptor.	bind
47849	2	10762	5	13	NULL	NULL	NULL	Nef receptor	GP		is a type of					death-signalling receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_422_3_363_s_108	9498817	A longer preincubation period for fasudil hydrochloride was required than for M3, probably because fasudil hydrochloride taken up by cells was converted to an active form M3 during this period [ 10], and thereby impeded transduction of the apoptosis-inducing signal introduced by binding of Nef to a putative Nef receptor, a death-signalling receptor.	bind
47851	3	10762	5	13	NULL	NULL	NULL	statement 1	Process		introduces					apoptosis-inducing signal	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_422_3_363_s_108	9498817	A longer preincubation period for fasudil hydrochloride was required than for M3, probably because fasudil hydrochloride taken up by cells was converted to an active form M3 during this period [ 10], and thereby impeded transduction of the apoptosis-inducing signal introduced by binding of Nef to a putative Nef receptor, a death-signalling receptor.	bind
47852	4	10762	5	13	NULL	NULL	NULL	fasudil hydrochloride	Chemical		is converted to					M3	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_422_3_363_s_108	9498817	A longer preincubation period for fasudil hydrochloride was required than for M3, probably because fasudil hydrochloride taken up by cells was converted to an active form M3 during this period [ 10], and thereby impeded transduction of the apoptosis-inducing signal introduced by binding of Nef to a putative Nef receptor, a death-signalling receptor.	bind
47853	5	10762	5	13	NULL	NULL	NULL	statement 4	Process		impede					apoptosis-inducing signal	Process	transduction of			NULL		NULL	NULL	NULL	NULL	gw60_febslett_422_3_363_s_108	9498817	A longer preincubation period for fasudil hydrochloride was required than for M3, probably because fasudil hydrochloride taken up by cells was converted to an active form M3 during this period [ 10], and thereby impeded transduction of the apoptosis-inducing signal introduced by binding of Nef to a putative Nef receptor, a death-signalling receptor.	bind
47317	1	10762	6	NULL	NULL	0	NULL	fasudil hydrochloride	NULL		is converted to	NULL				M3	NULL	active 			NULL		0	NULL	NULL	NULL	gw60_febslett_422_3_363_s_108	9498817	A longer preincubation period for fasudil hydrochloride was required than for M3, probably because fasudil hydrochloride taken up by cells was converted to an active form M3 during this period [ 10], and thereby impeded transduction of the apoptosis-inducing signal introduced by binding of Nef to a putative Nef receptor, a death-signalling receptor.	bind
47319	2	10762	6	NULL	NULL	0	NULL	Nef	NULL		bind	NULL				Nef receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_422_3_363_s_108	9498817	A longer preincubation period for fasudil hydrochloride was required than for M3, probably because fasudil hydrochloride taken up by cells was converted to an active form M3 during this period [ 10], and thereby impeded transduction of the apoptosis-inducing signal introduced by binding of Nef to a putative Nef receptor, a death-signalling receptor.	bind
47320	3	10762	6	NULL	NULL	0	NULL	Nef receptor	NULL		is a type of	NULL				death-signalling receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_422_3_363_s_108	9498817	A longer preincubation period for fasudil hydrochloride was required than for M3, probably because fasudil hydrochloride taken up by cells was converted to an active form M3 during this period [ 10], and thereby impeded transduction of the apoptosis-inducing signal introduced by binding of Nef to a putative Nef receptor, a death-signalling receptor.	bind
47323	4	10762	6	NULL	NULL	0	NULL	statement 2	NULL		introduces	NULL				apoptosis-inducing signal	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_422_3_363_s_108	9498817	A longer preincubation period for fasudil hydrochloride was required than for M3, probably because fasudil hydrochloride taken up by cells was converted to an active form M3 during this period [ 10], and thereby impeded transduction of the apoptosis-inducing signal introduced by binding of Nef to a putative Nef receptor, a death-signalling receptor.	bind
47326	5	10762	6	NULL	NULL	0	NULL	statement 1	NULL		impedes	NULL				apoptosis-inducing signal	NULL	transduction of 			NULL		0	NULL	NULL	NULL	gw60_febslett_422_3_363_s_108	9498817	A longer preincubation period for fasudil hydrochloride was required than for M3, probably because fasudil hydrochloride taken up by cells was converted to an active form M3 during this period [ 10], and thereby impeded transduction of the apoptosis-inducing signal introduced by binding of Nef to a putative Nef receptor, a death-signalling receptor.	bind
47850	1	10763	5	NULL	NULL	0	NULL		NULL		bind	NULL		Lys			NULL		S-adenosylmethionine		NULL		0	NULL	NULL	NULL	abs-batch0740-0759_plant-cell_18_7_16731588_s_7	16731588	A loop involved in the binding  of Lys and S-adenosylmethionine provides an explanation for the synergistic  inhibition by these effectors.	bind
47069	1	10763	6	NULL	NULL	0	NULL		NULL		bind	NULL		Lys			NULL		S-adenosylmethionine		NULL		0	NULL	NULL	NULL	abs-batch0740-0759_plant-cell_18_7_16731588_s_7	16731588	A loop involved in the binding  of Lys and S-adenosylmethionine provides an explanation for the synergistic  inhibition by these effectors.	bind
47854	1	10764	5	13	NULL	NULL	NULL	Brf1	GP		bind					TFIIIC-DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_172	16880507	A loop region in repeat II of the TFIIB homology domain is important for Brf1 binding  to TFIIIC-DNA.	bind
47855	2	10764	5	13	NULL	NULL	NULL	TFIIB	GP		is important for			loop region in repeat II of homology domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_172	16880507	A loop region in repeat II of the TFIIB homology domain is important for Brf1 binding  to TFIIIC-DNA.	bind
47070	1	10764	6	NULL	NULL	0	NULL	Brf1	NULL		bind	NULL				TFIIIC-DNA	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_172	16880507	A loop region in repeat II of the TFIIB homology domain is important for Brf1 binding  to TFIIIC-DNA.	bind
47071	2	10764	6	NULL	NULL	0	NULL	TFIIB	NULL		is important for	NULL		loop region in repeat II of homology domain		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_172	16880507	A loop region in repeat II of the TFIIB homology domain is important for Brf1 binding  to TFIIIC-DNA.	bind
47856	1	10765	5	NULL	NULL	0	NULL		NULL		bind	NULL		Arg-3500			NULL		Trp-4369		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_28_19732_s_250	16704977	A loop was proposed near the carboxyl-terminal end of apoB-100 ( ) that is stabilized by the binding of Arg-3500 to Trp-4369 ( ) and modulates the binding of the LDL receptor to the LDL receptor binding site (residues 3359-3369).	bind
47857	2	10765	5	13	NULL	NULL	NULL	statement 1	Process		stabilize					apoB-100	GP		loop near carboxyl-terminal end		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_28_19732_s_250	16704977	A loop was proposed near the carboxyl-terminal end of apoB-100 ( ) that is stabilized by the binding of Arg-3500 to Trp-4369 ( ) and modulates the binding of the LDL receptor to the LDL receptor binding site (residues 3359-3369).	bind
47858	3	10765	5	13	NULL	NULL	NULL	LDL receptor	GP		bind								LDL receptor binding site (3359-3369)		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_28_19732_s_250	16704977	A loop was proposed near the carboxyl-terminal end of apoB-100 ( ) that is stabilized by the binding of Arg-3500 to Trp-4369 ( ) and modulates the binding of the LDL receptor to the LDL receptor binding site (residues 3359-3369).	bind
47859	4	10765	5	13	NULL	NULL	NULL	apoB-100	GP	\t	modulates			loop near carboxyl-terminal end		statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_28_19732_s_250	16704977	A loop was proposed near the carboxyl-terminal end of apoB-100 ( ) that is stabilized by the binding of Arg-3500 to Trp-4369 ( ) and modulates the binding of the LDL receptor to the LDL receptor binding site (residues 3359-3369).	bind
47072	1	10765	6	NULL	NULL	0	NULL		NULL		bind	NULL		Arg-3500			NULL		Trp-4369		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_28_19732_s_250	16704977	A loop was proposed near the carboxyl-terminal end of apoB-100 ( ) that is stabilized by the binding of Arg-3500 to Trp-4369 ( ) and modulates the binding of the LDL receptor to the LDL receptor binding site (residues 3359-3369).	bind
47073	2	10765	6	NULL	NULL	0	NULL	LDL receptor	NULL		bind	NULL					NULL		 LDL receptor binding site		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_28_19732_s_250	16704977	A loop was proposed near the carboxyl-terminal end of apoB-100 ( ) that is stabilized by the binding of Arg-3500 to Trp-4369 ( ) and modulates the binding of the LDL receptor to the LDL receptor binding site (residues 3359-3369).	bind
47074	3	10765	6	NULL	NULL	0	NULL	apoB-100	NULL		is stabilized by	NULL		loop near carboxyl-terminal end		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_28_19732_s_250	16704977	A loop was proposed near the carboxyl-terminal end of apoB-100 ( ) that is stabilized by the binding of Arg-3500 to Trp-4369 ( ) and modulates the binding of the LDL receptor to the LDL receptor binding site (residues 3359-3369).	bind
47075	4	10765	6	NULL	NULL	0	NULL	apoB-100	NULL		modulates	NULL		loop near carboxyl-terminal end		statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_28_19732_s_250	16704977	A loop was proposed near the carboxyl-terminal end of apoB-100 ( ) that is stabilized by the binding of Arg-3500 to Trp-4369 ( ) and modulates the binding of the LDL receptor to the LDL receptor binding site (residues 3359-3369).	bind
47076	5	10765	6	NULL	NULL	0	NULL	LDL receptor binding site	NULL		resides between	NULL				residues 3359-3369	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_28_19732_s_250	16704977	A loop was proposed near the carboxyl-terminal end of apoB-100 ( ) that is stabilized by the binding of Arg-3500 to Trp-4369 ( ) and modulates the binding of the LDL receptor to the LDL receptor binding site (residues 3359-3369).	bind
47919	1	10766	5	13	NULL	NULL	NULL	Brf1	GP		bind					TFIIIC	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_345	16880507	A loss-of-function mutation in TPR7 (L469K) of Tfc4 was previously shown to decrease Brf1 (and Bdp1) binding to TFIIIC.	bind
47920	2	10766	5	13	NULL	NULL	NULL	Bdp1	GP		bind					TFIIIC	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_345	16880507	A loss-of-function mutation in TPR7 (L469K) of Tfc4 was previously shown to decrease Brf1 (and Bdp1) binding to TFIIIC.	bind
47921	3	10766	5	13	NULL	NULL	NULL	Tfc4	GP	mutant	decreases			TPR7 (L469K)		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_345	16880507	A loss-of-function mutation in TPR7 (L469K) of Tfc4 was previously shown to decrease Brf1 (and Bdp1) binding to TFIIIC.	bind
47922	4	10766	5	13	NULL	NULL	NULL	Tfc4	GP	mutant	decreases			TPR7 (L469K)		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_345	16880507	A loss-of-function mutation in TPR7 (L469K) of Tfc4 was previously shown to decrease Brf1 (and Bdp1) binding to TFIIIC.	bind
47119	1	10766	6	NULL	NULL	0	NULL	Brf1	NULL		bind	NULL				TFIIIC	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_345	16880507	A loss-of-function mutation in TPR7 (L469K) of Tfc4 was previously shown to decrease Brf1 (and Bdp1) binding to TFIIIC.	bind
47120	2	10766	6	NULL	NULL	0	NULL	Bdp1	NULL		bind	NULL				TFIIIC	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_345	16880507	A loss-of-function mutation in TPR7 (L469K) of Tfc4 was previously shown to decrease Brf1 (and Bdp1) binding to TFIIIC.	bind
47124	3	10766	6	NULL	NULL	0	NULL	Tfc4	NULL	mutant	decreases	NULL		L469K in TPR7		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_345	16880507	A loss-of-function mutation in TPR7 (L469K) of Tfc4 was previously shown to decrease Brf1 (and Bdp1) binding to TFIIIC.	bind
47125	4	10766	6	NULL	NULL	0	NULL	Tfc4	NULL	mutant	decreases	NULL		L469K in TPR7		statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_345	16880507	A loss-of-function mutation in TPR7 (L469K) of Tfc4 was previously shown to decrease Brf1 (and Bdp1) binding to TFIIIC.	bind
47923	1	10767	5	13	NULL	NULL	NULL	NS1	Organism		bind		inefficient			NS2	Organism				NULL		NULL	NULL	NULL	NULL	gw70_femsimmunolmedmic_35_2_87_s_108	12628542	A low adsorption rate due to inefficient binding of NS1 and NS2 might also result  in failure to detect phage susceptibility.	bind
47126	1	10767	6	NULL	NULL	0	NULL	NS1	NULL		bind	NULL	inefficiently			NS2	NULL				NULL		0	NULL	NULL	NULL	gw70_femsimmunolmedmic_35_2_87_s_108	12628542	A low adsorption rate due to inefficient binding of NS1 and NS2 might also result  in failure to detect phage susceptibility.	bind
47924	1	10769	5	13	NULL	NULL	NULL	Fas	GP		bind		low affinity			UBC-FAP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_49_31037_s_224	8940097	A low binding affinity between Fas and UBC-FAP may explain our unsuccessful efforts to date to coprecipitate these proteins from cell lysates.	bind
47127	1	10769	6	NULL	NULL	0	NULL	Fas	NULL		bind	NULL	low affinity			UBC-FAP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_49_31037_s_224	8940097	A low binding affinity between Fas and UBC-FAP may explain our unsuccessful efforts to date to coprecipitate these proteins from cell lysates.	bind
47925	1	10770	5	13	NULL	NULL	NULL	APC	GP		bind					EPCR	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_29_20077_s_130	16709569	A low concentration of exogenous APC (3.3 nM) was used, and barrier protective effects of exogenous APC were blocked by both wild type PC and PC S360A, consistent with the expected role of zymogen PC as a competitive inhibitor for APC binding to EPCR.	bind
47926	2	10770	5	13	NULL	NULL	NULL	zymogen PC	GP		bind					EPCR	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_29_20077_s_130	16709569	A low concentration of exogenous APC (3.3 nM) was used, and barrier protective effects of exogenous APC were blocked by both wild type PC and PC S360A, consistent with the expected role of zymogen PC as a competitive inhibitor for APC binding to EPCR.	bind
47927	3	10770	5	13	NULL	NULL	NULL	APC	GP	exogenous	effects					barrier protective	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_29_20077_s_130	16709569	A low concentration of exogenous APC (3.3 nM) was used, and barrier protective effects of exogenous APC were blocked by both wild type PC and PC S360A, consistent with the expected role of zymogen PC as a competitive inhibitor for APC binding to EPCR.	bind
47928	4	10770	5	13	NULL	NULL	NULL	PC	GP	wild type	blocks					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_29_20077_s_130	16709569	A low concentration of exogenous APC (3.3 nM) was used, and barrier protective effects of exogenous APC were blocked by both wild type PC and PC S360A, consistent with the expected role of zymogen PC as a competitive inhibitor for APC binding to EPCR.	bind
47929	5	10770	5	13	NULL	NULL	NULL	PC	GP		blocks			S360A		statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_29_20077_s_130	16709569	A low concentration of exogenous APC (3.3 nM) was used, and barrier protective effects of exogenous APC were blocked by both wild type PC and PC S360A, consistent with the expected role of zymogen PC as a competitive inhibitor for APC binding to EPCR.	bind
50358	6	10770	5	13	NULL	NULL	NULL	statement 1	Process		compete with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_29_20077_s_130	16709569	A low concentration of exogenous APC (3.3 nM) was used, and barrier protective effects of exogenous APC were blocked by both wild type PC and PC S360A, consistent with the expected role of zymogen PC as a competitive inhibitor for APC binding to EPCR.	bind
47274	1	10770	6	NULL	NULL	0	NULL	APC	NULL		bind	NULL				EPCR	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_29_20077_s_130	16709569	A low concentration of exogenous APC (3.3 nM) was used, and barrier protective effects of exogenous APC were blocked by both wild type PC and PC S360A, consistent with the expected role of zymogen PC as a competitive inhibitor for APC binding to EPCR.	bind
47276	2	10770	6	NULL	NULL	0	NULL	zymogen PC	NULL		bind	NULL				EPCR	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_29_20077_s_130	16709569	A low concentration of exogenous APC (3.3 nM) was used, and barrier protective effects of exogenous APC were blocked by both wild type PC and PC S360A, consistent with the expected role of zymogen PC as a competitive inhibitor for APC binding to EPCR.	bind
47278	3	10770	6	NULL	NULL	0	NULL	statement 1	NULL		competes	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_29_20077_s_130	16709569	A low concentration of exogenous APC (3.3 nM) was used, and barrier protective effects of exogenous APC were blocked by both wild type PC and PC S360A, consistent with the expected role of zymogen PC as a competitive inhibitor for APC binding to EPCR.	bind
47279	4	10770	6	10	NULL	0	NULL	APC		exogenous	effects					barrier protective					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_29_20077_s_130	16709569	A low concentration of exogenous APC (3.3 nM) was used, and barrier protective effects of exogenous APC were blocked by both wild type PC and PC S360A, consistent with the expected role of zymogen PC as a competitive inhibitor for APC binding to EPCR.	bind
47280	5	10770	6	NULL	NULL	0	NULL	statement 4	NULL		is blocked by	NULL				PC	NULL	wild type			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_29_20077_s_130	16709569	A low concentration of exogenous APC (3.3 nM) was used, and barrier protective effects of exogenous APC were blocked by both wild type PC and PC S360A, consistent with the expected role of zymogen PC as a competitive inhibitor for APC binding to EPCR.	bind
47281	6	10770	6	NULL	NULL	0	NULL	statement 4	NULL		is blocked by	NULL				PC	NULL		S360A		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_29_20077_s_130	16709569	A low concentration of exogenous APC (3.3 nM) was used, and barrier protective effects of exogenous APC were blocked by both wild type PC and PC S360A, consistent with the expected role of zymogen PC as a competitive inhibitor for APC binding to EPCR.	bind
47930	1	10774	5	13	NULL	NULL	NULL				bind				CSL-binding site in the GC-rich domain	Notch 1	GP		ICD		NULL		NULL	NULL	NULL	NULL	gw70_development_130_24_6089_s_198	14597575	A low level of induction was also observed with Notch 1 ICD alone ( Fig. 6B), suggesting that the CSL-binding site in the GC-rich domain could bind Notch 1 ICD through CSL.	bind
57236	2	10774	5	13	NULL	NULL	NULL	statement 1	Process		occurs through					CSL	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_130_24_6089_s_198	14597575	A low level of induction was also observed with Notch 1 ICD alone ( Fig. 6B), suggesting that the CSL-binding site in the GC-rich domain could bind Notch 1 ICD through CSL.	bind
47128	1	10774	6	NULL	NULL	0	NULL	Notch 1	NULL		bind	NULL		ICD		CSL	NULL		CSL-binding site in the GC-rich domain		NULL		0	NULL	NULL	NULL	gw70_development_130_24_6089_s_198	14597575	A low level of induction was also observed with Notch 1 ICD alone ( Fig. 6B), suggesting that the CSL-binding site in the GC-rich domain could bind Notch 1 ICD through CSL.	bind
57237	2	10774	6	10	NULL	0	NULL	statement 1			occurs through					CSL					NULL		0	NULL	NULL	NULL	gw70_development_130_24_6089_s_198	14597575	A low level of induction was also observed with Notch 1 ICD alone ( Fig. 6B), suggesting that the CSL-binding site in the GC-rich domain could bind Notch 1 ICD through CSL.	bind
47932	1	10775	5	13	NULL	NULL	NULL	PP1	GP		bind					PNUTS	GP		309-401		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_16_13819_s_140	12574161	A low level of PP1 was found to bind to PNUTS-(309-401), but no binding was detected for PNUTS-(404-537), PNUTS-(590-872), and PNUTS-(724-872) or for two fragments with an internal deletion of residues 254-589.	bind
47933	2	10775	5	13	NULL	NULL	NULL	PP1	GP		does not bind					PNUTS	GP		404-537		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_16_13819_s_140	12574161	A low level of PP1 was found to bind to PNUTS-(309-401), but no binding was detected for PNUTS-(404-537), PNUTS-(590-872), and PNUTS-(724-872) or for two fragments with an internal deletion of residues 254-589.	bind
47934	3	10775	5	13	NULL	NULL	NULL	PP1	GP		does not bind					PNUTS	GP		590-872		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_16_13819_s_140	12574161	A low level of PP1 was found to bind to PNUTS-(309-401), but no binding was detected for PNUTS-(404-537), PNUTS-(590-872), and PNUTS-(724-872) or for two fragments with an internal deletion of residues 254-589.	bind
47935	4	10775	5	13	NULL	NULL	NULL	PP1	GP		does not bind					PNUTS	GP		724-872		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_16_13819_s_140	12574161	A low level of PP1 was found to bind to PNUTS-(309-401), but no binding was detected for PNUTS-(404-537), PNUTS-(590-872), and PNUTS-(724-872) or for two fragments with an internal deletion of residues 254-589.	bind
47129	1	10775	6	NULL	NULL	0	NULL	PP1	NULL		bind	NULL				PNUTS	NULL		309-401		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_16_13819_s_140	12574161	A low level of PP1 was found to bind to PNUTS-(309-401), but no binding was detected for PNUTS-(404-537), PNUTS-(590-872), and PNUTS-(724-872) or for two fragments with an internal deletion of residues 254-589.	bind
47130	2	10775	6	NULL	NULL	0	NULL	PP1	NULL		does not bind	NULL				PNUTS	NULL		404-537		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_16_13819_s_140	12574161	A low level of PP1 was found to bind to PNUTS-(309-401), but no binding was detected for PNUTS-(404-537), PNUTS-(590-872), and PNUTS-(724-872) or for two fragments with an internal deletion of residues 254-589.	bind
47131	3	10775	6	NULL	NULL	0	NULL	PP1	NULL		does not bind	NULL				PNUTS	NULL		724-872		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_16_13819_s_140	12574161	A low level of PP1 was found to bind to PNUTS-(309-401), but no binding was detected for PNUTS-(404-537), PNUTS-(590-872), and PNUTS-(724-872) or for two fragments with an internal deletion of residues 254-589.	bind
47132	4	10775	6	NULL	NULL	0	NULL	PP1	NULL		does not bind	NULL				PNUTS	NULL		590-872		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_16_13819_s_140	12574161	A low level of PP1 was found to bind to PNUTS-(309-401), but no binding was detected for PNUTS-(404-537), PNUTS-(590-872), and PNUTS-(724-872) or for two fragments with an internal deletion of residues 254-589.	bind
47936	1	10776	5	13	NULL	NULL	NULL	Sba1p	GP		bind					GR	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_4_422_s_76	10691735	A low level of Sba1p reproducibly remained bound to GR and MR after hormone addition, possibly indicating that p23 proteins might affect both holoreceptors and aporeceptors.	bind
47937	2	10776	5	13	NULL	NULL	NULL	Sba1p	GP		bind					MR	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_4_422_s_76	10691735	A low level of Sba1p reproducibly remained bound to GR and MR after hormone addition, possibly indicating that p23 proteins might affect both holoreceptors and aporeceptors.	bind
47938	3	10776	5	13	NULL	NULL	NULL	hormone	Chemical	addition of	retains					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_4_422_s_76	10691735	A low level of Sba1p reproducibly remained bound to GR and MR after hormone addition, possibly indicating that p23 proteins might affect both holoreceptors and aporeceptors.	bind
47939	4	10776	5	13	NULL	NULL	NULL	hormone	Chemical	addition of	retains					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_4_422_s_76	10691735	A low level of Sba1p reproducibly remained bound to GR and MR after hormone addition, possibly indicating that p23 proteins might affect both holoreceptors and aporeceptors.	bind
47940	5	10776	5	13	NULL	NULL	NULL	p23 proteins	GP		effect		might			holoreceptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_4_422_s_76	10691735	A low level of Sba1p reproducibly remained bound to GR and MR after hormone addition, possibly indicating that p23 proteins might affect both holoreceptors and aporeceptors.	bind
47941	6	10776	5	13	NULL	NULL	NULL	p23 proteins	GP		effect		might			aporeceptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_4_422_s_76	10691735	A low level of Sba1p reproducibly remained bound to GR and MR after hormone addition, possibly indicating that p23 proteins might affect both holoreceptors and aporeceptors.	bind
47152	1	10776	6	NULL	NULL	0	NULL	Sba1p	NULL		bind	NULL				GR	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_14_4_422_s_76	10691735	A low level of Sba1p reproducibly remained bound to GR and MR after hormone addition, possibly indicating that p23 proteins might affect both holoreceptors and aporeceptors.	bind
47153	2	10776	6	NULL	NULL	0	NULL	Sba1p	NULL		bind	NULL				MR	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_14_4_422_s_76	10691735	A low level of Sba1p reproducibly remained bound to GR and MR after hormone addition, possibly indicating that p23 proteins might affect both holoreceptors and aporeceptors.	bind
47156	3	10776	6	10	NULL	0	NULL	p23 protein			affect		might			holoreceptors					NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_4_422_s_76	10691735	A low level of Sba1p reproducibly remained bound to GR and MR after hormone addition, possibly indicating that p23 proteins might affect both holoreceptors and aporeceptors.	bind
47157	4	10776	6	10	NULL	0	NULL	p23 protein			affects		might			aporeceptors					NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_4_422_s_76	10691735	A low level of Sba1p reproducibly remained bound to GR and MR after hormone addition, possibly indicating that p23 proteins might affect both holoreceptors and aporeceptors.	bind
50359	5	10776	6	10	NULL	0	NULL	hormone	NULL	addition of	retains	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_14_4_422_s_76	10691735	A low level of Sba1p reproducibly remained bound to GR and MR after hormone addition, possibly indicating that p23 proteins might affect both holoreceptors and aporeceptors.	bind
50360	6	10776	6	10	NULL	0	NULL	hormone	NULL	addition of	retains	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_14_4_422_s_76	10691735	A low level of Sba1p reproducibly remained bound to GR and MR after hormone addition, possibly indicating that p23 proteins might affect both holoreceptors and aporeceptors.	bind
47942	1	10777	5	13	NULL	NULL	NULL	PapI	GP		is a type of					coregulatory protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_70_3_830_s_307	16959970	A low level of the coregulatory protein PapI, required for Pap pili expression ( ,  ,  ), increases the affinity of Lrp for  pap DNA hemimethylated at GATCdist but does not enhance binding of Lrp to  pap DNA fully methylated at GATCdist ( ).	bind
47943	2	10777	5	13	NULL	NULL	NULL	PapI	GP		is required for					Pap pili	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_70_3_830_s_307	16959970	A low level of the coregulatory protein PapI, required for Pap pili expression ( ,  ,  ), increases the affinity of Lrp for  pap DNA hemimethylated at GATCdist but does not enhance binding of Lrp to  pap DNA fully methylated at GATCdist ( ).	bind
47944	3	10777	5	13	NULL	NULL	NULL	Lrp	GP		shows affinity to					pap DNA	NucleicAcid	hemimethylated		GATCdist	NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_70_3_830_s_307	16959970	A low level of the coregulatory protein PapI, required for Pap pili expression ( ,  ,  ), increases the affinity of Lrp for  pap DNA hemimethylated at GATCdist but does not enhance binding of Lrp to  pap DNA fully methylated at GATCdist ( ).	bind
47945	4	10777	5	13	NULL	NULL	NULL	Lrp	GP		bind					pap DNA	NucleicAcid	fully methylated		GATCdist	NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_70_3_830_s_307	16959970	A low level of the coregulatory protein PapI, required for Pap pili expression ( ,  ,  ), increases the affinity of Lrp for  pap DNA hemimethylated at GATCdist but does not enhance binding of Lrp to  pap DNA fully methylated at GATCdist ( ).	bind
47946	5	10777	5	13	NULL	NULL	NULL	PapI	GP		increases					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_70_3_830_s_307	16959970	A low level of the coregulatory protein PapI, required for Pap pili expression ( ,  ,  ), increases the affinity of Lrp for  pap DNA hemimethylated at GATCdist but does not enhance binding of Lrp to  pap DNA fully methylated at GATCdist ( ).	bind
47947	6	10777	5	13	NULL	NULL	NULL	PapI	GP		does not enhance					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_70_3_830_s_307	16959970	A low level of the coregulatory protein PapI, required for Pap pili expression ( ,  ,  ), increases the affinity of Lrp for  pap DNA hemimethylated at GATCdist but does not enhance binding of Lrp to  pap DNA fully methylated at GATCdist ( ).	bind
47329	1	10777	6	NULL	NULL	0	NULL	PapI	NULL		is a type of	NULL				coregulatory protein	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_70_3_830_s_307	16959970	A low level of the coregulatory protein PapI, required for Pap pili expression ( ,  ,  ), increases the affinity of Lrp for  pap DNA hemimethylated at GATCdist but does not enhance binding of Lrp to  pap DNA fully methylated at GATCdist ( ).	bind
47330	2	10777	6	NULL	NULL	0	NULL	PapI	NULL		is required for	NULL				Pap pili	NULL	expression of 			NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_70_3_830_s_307	16959970	A low level of the coregulatory protein PapI, required for Pap pili expression ( ,  ,  ), increases the affinity of Lrp for  pap DNA hemimethylated at GATCdist but does not enhance binding of Lrp to  pap DNA fully methylated at GATCdist ( ).	bind
47331	3	10777	6	10	NULL	0	NULL	Lrp	NULL		shows affinity to	NULL				pap DNA	NULL	hemimethylated		GATCdist	NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_70_3_830_s_307	16959970	A low level of the coregulatory protein PapI, required for Pap pili expression ( ,  ,  ), increases the affinity of Lrp for  pap DNA hemimethylated at GATCdist but does not enhance binding of Lrp to  pap DNA fully methylated at GATCdist ( ).	bind
47335	4	10777	6	10	NULL	0	NULL	Lrp	NULL		shows affinity to	NULL				pap DNA	NULL	fully methylated		GATCdist	NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_70_3_830_s_307	16959970	A low level of the coregulatory protein PapI, required for Pap pili expression ( ,  ,  ), increases the affinity of Lrp for  pap DNA hemimethylated at GATCdist but does not enhance binding of Lrp to  pap DNA fully methylated at GATCdist ( ).	bind
47337	5	10777	6	10	NULL	0	NULL	PapI	NULL		increase	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_70_3_830_s_307	16959970	A low level of the coregulatory protein PapI, required for Pap pili expression ( ,  ,  ), increases the affinity of Lrp for  pap DNA hemimethylated at GATCdist but does not enhance binding of Lrp to  pap DNA fully methylated at GATCdist ( ).	bind
50361	6	10777	6	10	NULL	0	NULL	PapI	NULL		does not enhance	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_70_3_830_s_307	16959970	A low level of the coregulatory protein PapI, required for Pap pili expression ( ,  ,  ), increases the affinity of Lrp for  pap DNA hemimethylated at GATCdist but does not enhance binding of Lrp to  pap DNA fully methylated at GATCdist ( ).	bind
47948	1	10779	5	13	NULL	NULL	NULL	retinol binding protein	GP		bind					transthyretin	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevnutr_21_0_167_s_802	11375434	A low molar ratio of retinol binding protein to transthyretin  indicates vitamin A deficiency during inflammation: studies in rats and a posterior  analysis of vitamin A-supplemented children with measles.	bind
47949	2	10779	5	13	NULL	NULL	NULL	statement 1	Process		indicates					vitamin A	Chemical	deficiency of			NULL		NULL	NULL	NULL	NULL	gw70_annurevnutr_21_0_167_s_802	11375434	A low molar ratio of retinol binding protein to transthyretin  indicates vitamin A deficiency during inflammation: studies in rats and a posterior  analysis of vitamin A-supplemented children with measles.	bind
47950	3	10779	5	13	NULL	NULL	NULL	statement 2	GP		occurs during					inflammation	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevnutr_21_0_167_s_802	11375434	A low molar ratio of retinol binding protein to transthyretin  indicates vitamin A deficiency during inflammation: studies in rats and a posterior  analysis of vitamin A-supplemented children with measles.	bind
47174	1	10779	6	NULL	NULL	0	NULL	retinol binding protein	NULL		bind	NULL	low affinity			transthyretin	NULL				NULL		NULL	NULL	NULL	NULL	gw70_annurevnutr_21_0_167_s_802	11375434	A low molar ratio of retinol binding protein to transthyretin  indicates vitamin A deficiency during inflammation: studies in rats and a posterior  analysis of vitamin A-supplemented children with measles.	bind
47175	2	10779	6	NULL	NULL	0	NULL	statement 1	NULL		indicates	NULL				vitamin A	NULL	deficiency of			NULL		0	NULL	NULL	NULL	gw70_annurevnutr_21_0_167_s_802	11375434	A low molar ratio of retinol binding protein to transthyretin  indicates vitamin A deficiency during inflammation: studies in rats and a posterior  analysis of vitamin A-supplemented children with measles.	bind
47176	3	10779	6	NULL	NULL	0	NULL	statement 2	NULL		occurs during 	NULL				inflammation	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevnutr_21_0_167_s_802	11375434	A low molar ratio of retinol binding protein to transthyretin  indicates vitamin A deficiency during inflammation: studies in rats and a posterior  analysis of vitamin A-supplemented children with measles.	bind
47951	1	10780	5	13	NULL	NULL	NULL	CXCL12	GP	labeled	bind					CXCR4	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_eur-cytokine-netw_17_1_16613763_s_7	16613763	A low molecular weight antagonist of CXCR4 prevented binding of labeled  CXCL12 to CXCR4 comparably to a neutralizing anti-CXCR4 antibody.	bind
47952	2	10780	5	13	NULL	NULL	NULL	CXCR4 antagonist	Chemical	low molecular weight	prevents					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_eur-cytokine-netw_17_1_16613763_s_7	16613763	A low molecular weight antagonist of CXCR4 prevented binding of labeled  CXCL12 to CXCR4 comparably to a neutralizing anti-CXCR4 antibody.	bind
47177	1	10780	6	NULL	NULL	0	NULL	CXCL12	NULL	labeled	bind	NULL				CXCR4	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_eur-cytokine-netw_17_1_16613763_s_7	16613763	A low molecular weight antagonist of CXCR4 prevented binding of labeled  CXCL12 to CXCR4 comparably to a neutralizing anti-CXCR4 antibody.	bind
47178	2	10780	6	NULL	NULL	0	NULL	CXCR4 antagonist	NULL	low molecular weight	prevents	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_eur-cytokine-netw_17_1_16613763_s_7	16613763	A low molecular weight antagonist of CXCR4 prevented binding of labeled  CXCL12 to CXCR4 comparably to a neutralizing anti-CXCR4 antibody.	bind
47953	1	10781	5	13	NULL	NULL	NULL	12 antenna Chls	Chemical	S. elongatus	bind					CP43	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_530_1_117_s_164	12387877	A low resolution (3.8  Ang ) X-ray crystal structure for this complex from  S. elongatus has been described [ 4, that included 12 antenna Chls bound to CP43 and 14 antenna Chls bound to CP47.	bind
47954	2	10781	5	13	NULL	NULL	NULL	14 antenna Chls	Chemical	S. elongatus	bind					CP47	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_530_1_117_s_164	12387877	A low resolution (3.8  Ang ) X-ray crystal structure for this complex from  S. elongatus has been described [ 4, that included 12 antenna Chls bound to CP43 and 14 antenna Chls bound to CP47.	bind
47179	1	10781	6	NULL	NULL	0	NULL	12 antenna Chls	NULL	S. elongatus	bind	NULL				CP43	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_530_1_117_s_164	12387877	A low resolution (3.8  Ang ) X-ray crystal structure for this complex from  S. elongatus has been described [ 4, that included 12 antenna Chls bound to CP43 and 14 antenna Chls bound to CP47.	bind
47180	2	10781	6	NULL	NULL	0	NULL	14 antenna Chls	NULL	S. elongatus	bind	NULL				CP47	NULL				NULL		NULL	NULL	NULL	NULL	gw60_febslett_530_1_117_s_164	12387877	A low resolution (3.8  Ang ) X-ray crystal structure for this complex from  S. elongatus has been described [ 4, that included 12 antenna Chls bound to CP43 and 14 antenna Chls bound to CP47.	bind
47958	1	10782	5	13	NULL	NULL	NULL	atherosclerosis	Process	low risk of	is observed in					APOB	GP	mutation of	LDL binding region		NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_7_693_s_20	10449689	A low risk of atherosclerosis is observed in  APOB mutations outside the LDL binding region and in cholesteryl ester transfer protein ( CETP) deficiency, whereas the impact of  APOAII deficiency on atherosclerosis has not been established 1  (Table 1  ).	bind
47959	2	10782	5	13	NULL	NULL	NULL	atherosclerosis	Process	low risk of	is observed in					CETP	GP	deficiency of			NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_7_693_s_20	10449689	A low risk of atherosclerosis is observed in  APOB mutations outside the LDL binding region and in cholesteryl ester transfer protein ( CETP) deficiency, whereas the impact of  APOAII deficiency on atherosclerosis has not been established 1  (Table 1  ).	bind
47960	3	10782	5	13	NULL	NULL	NULL	CETP	GP		is					cholesteryl ester transfer protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_100_7_693_s_20	10449689	A low risk of atherosclerosis is observed in  APOB mutations outside the LDL binding region and in cholesteryl ester transfer protein ( CETP) deficiency, whereas the impact of  APOAII deficiency on atherosclerosis has not been established 1  (Table 1  ).	bind
47349	1	10782	6	NULL	NULL	0	NULL	CETP	NULL		is	NULL				cholesteryl ester transfer protein	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_100_7_693_s_20	10449689	A low risk of atherosclerosis is observed in  APOB mutations outside the LDL binding region and in cholesteryl ester transfer protein ( CETP) deficiency, whereas the impact of  APOAII deficiency on atherosclerosis has not been established 1  (Table 1  ).	bind
47350	2	10782	6	NULL	NULL	0	NULL	CETP	NULL	deficiency of	causes risk of	NULL				atherosclerosis	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_100_7_693_s_20	10449689	A low risk of atherosclerosis is observed in  APOB mutations outside the LDL binding region and in cholesteryl ester transfer protein ( CETP) deficiency, whereas the impact of  APOAII deficiency on atherosclerosis has not been established 1  (Table 1  ).	bind
47351	3	10782	6	NULL	NULL	0	NULL	APOB	NULL	mutation of	causes risk of	NULL	low	LDL binding region		atherosclerosis	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_100_7_693_s_20	10449689	A low risk of atherosclerosis is observed in  APOB mutations outside the LDL binding region and in cholesteryl ester transfer protein ( CETP) deficiency, whereas the impact of  APOAII deficiency on atherosclerosis has not been established 1  (Table 1  ).	bind
47961	1	10783	5	13	NULL	NULL	NULL	seminal plasma	Chemical	human;;low-molecular-weight fraction of	activates					adenylyl cyclase	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5385_2027_s_405	9748162	A low-molecular-weight fraction of human seminal plasma activates adenylyl cyclase and induces caspase 3-independent apoptosis in prostatic epithelial cells by decreasing mitochondrial potential and Bcl-2/Bax ratio.	bind
47962	2	10783	5	13	NULL	NULL	NULL	apoptosis	GP		is independent of					caspase 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5385_2027_s_405	9748162	A low-molecular-weight fraction of human seminal plasma activates adenylyl cyclase and induces caspase 3-independent apoptosis in prostatic epithelial cells by decreasing mitochondrial potential and Bcl-2/Bax ratio.	bind
47963	3	10783	5	13	NULL	NULL	NULL	statement 1	Process		induces					statement 2	Process				NULL	prostatic epithelial cells	NULL	NULL	NULL	NULL	gw60_science_281_5385_2027_s_405	9748162	A low-molecular-weight fraction of human seminal plasma activates adenylyl cyclase and induces caspase 3-independent apoptosis in prostatic epithelial cells by decreasing mitochondrial potential and Bcl-2/Bax ratio.	bind
47964	4	10783	5	13	NULL	NULL	NULL	statement 3	Process		occurs by					mitochondrial potential	Process	decreasing			NULL		NULL	NULL	NULL	NULL	gw60_science_281_5385_2027_s_405	9748162	A low-molecular-weight fraction of human seminal plasma activates adenylyl cyclase and induces caspase 3-independent apoptosis in prostatic epithelial cells by decreasing mitochondrial potential and Bcl-2/Bax ratio.	bind
47965	5	10783	5	13	NULL	NULL	NULL	statement 3	Process		occurs by					Bcl-2/Bax ratio	GP	decreasing			NULL		NULL	NULL	NULL	NULL	gw60_science_281_5385_2027_s_405	9748162	A low-molecular-weight fraction of human seminal plasma activates adenylyl cyclase and induces caspase 3-independent apoptosis in prostatic epithelial cells by decreasing mitochondrial potential and Bcl-2/Bax ratio.	bind
47181	1	10783	6	NULL	NULL	0	NULL	seminal plasma	NULL	human;; low molecular weight fraction of	activates	NULL				adenylyl cyclase	NULL				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5385_2027_s_405	9748162	A low-molecular-weight fraction of human seminal plasma activates adenylyl cyclase and induces caspase 3-independent apoptosis in prostatic epithelial cells by decreasing mitochondrial potential and Bcl-2/Bax ratio.	bind
47182	2	10783	6	NULL	NULL	0	NULL	apoptosis	NULL		is independent of	NULL				caspase-3	NULL				NULL		0	NULL	NULL	NULL	gw60_science_281_5385_2027_s_405	9748162	A low-molecular-weight fraction of human seminal plasma activates adenylyl cyclase and induces caspase 3-independent apoptosis in prostatic epithelial cells by decreasing mitochondrial potential and Bcl-2/Bax ratio.	bind
47183	3	10783	6	NULL	NULL	0	NULL	statement 1	NULL		induces	NULL				statement 2	NULL				NULL	prostatic epithelial cells	0	NULL	NULL	NULL	gw60_science_281_5385_2027_s_405	9748162	A low-molecular-weight fraction of human seminal plasma activates adenylyl cyclase and induces caspase 3-independent apoptosis in prostatic epithelial cells by decreasing mitochondrial potential and Bcl-2/Bax ratio.	bind
47184	4	10783	6	NULL	NULL	0	NULL	statement 3	NULL		occurs by	NULL				mitochondrial potential	NULL	decreasing			NULL		0	NULL	NULL	NULL	gw60_science_281_5385_2027_s_405	9748162	A low-molecular-weight fraction of human seminal plasma activates adenylyl cyclase and induces caspase 3-independent apoptosis in prostatic epithelial cells by decreasing mitochondrial potential and Bcl-2/Bax ratio.	bind
47185	5	10783	6	NULL	NULL	0	NULL	statement 3	NULL		occurs by	NULL				Bcl-2/Bax ratio	NULL	decreasing			NULL		0	NULL	NULL	NULL	gw60_science_281_5385_2027_s_405	9748162	A low-molecular-weight fraction of human seminal plasma activates adenylyl cyclase and induces caspase 3-independent apoptosis in prostatic epithelial cells by decreasing mitochondrial potential and Bcl-2/Bax ratio.	bind
47966	1	10784	5	13	NULL	NULL	NULL	BD-Pdcd4	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_9_3894_s_68	15082783	A luciferase reporter becomes activated when the BD-Pdcd4 (wild-type or mutant) fusion protein binds to the AD-eIF4A fusion protein.	bind
47967	2	10784	5	13	NULL	NULL	NULL	AD-eIF4A	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_9_3894_s_68	15082783	A luciferase reporter becomes activated when the BD-Pdcd4 (wild-type or mutant) fusion protein binds to the AD-eIF4A fusion protein.	bind
47968	3	10784	5	13	NULL	NULL	NULL	BD-Pdcd4	GP	wild-type	bind					AD-eIF4A	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_9_3894_s_68	15082783	A luciferase reporter becomes activated when the BD-Pdcd4 (wild-type or mutant) fusion protein binds to the AD-eIF4A fusion protein.	bind
47969	4	10784	5	13	NULL	NULL	NULL	BD-Pdcd4	GP	mutant	bind					AD-eIF4A	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_9_3894_s_68	15082783	A luciferase reporter becomes activated when the BD-Pdcd4 (wild-type or mutant) fusion protein binds to the AD-eIF4A fusion protein.	bind
47970	5	10784	5	13	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_9_3894_s_68	15082783	A luciferase reporter becomes activated when the BD-Pdcd4 (wild-type or mutant) fusion protein binds to the AD-eIF4A fusion protein.	bind
47186	1	10784	6	10	NULL	0	NULL	BD-Pdcd4	NULL	wild type	bind	NULL				AD-eIF4A	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_9_3894_s_68	15082783	A luciferase reporter becomes activated when the BD-Pdcd4 (wild-type or mutant) fusion protein binds to the AD-eIF4A fusion protein.	bind
47187	2	10784	6	10	NULL	0	NULL	BD-Pdcd4 	NULL	mutant	bind	NULL				AD-eIF4A	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_9_3894_s_68	15082783	A luciferase reporter becomes activated when the BD-Pdcd4 (wild-type or mutant) fusion protein binds to the AD-eIF4A fusion protein.	bind
47188	3	10784	6	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_9_3894_s_68	15082783	A luciferase reporter becomes activated when the BD-Pdcd4 (wild-type or mutant) fusion protein binds to the AD-eIF4A fusion protein.	bind
50362	4	10784	6	10	NULL	0	NULL	BD-Pdcd4	NULL		is a type of	NULL				fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_9_3894_s_68	15082783	A luciferase reporter becomes activated when the BD-Pdcd4 (wild-type or mutant) fusion protein binds to the AD-eIF4A fusion protein.	bind
50363	5	10784	6	10	NULL	0	NULL	AD-eIF4A	NULL		is a type of	NULL				fusion protein	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_9_3894_s_68	15082783	A luciferase reporter becomes activated when the BD-Pdcd4 (wild-type or mutant) fusion protein binds to the AD-eIF4A fusion protein.	bind
47971	1	10785	5	13	NULL	NULL	NULL	HsCdc6	GP		forms complex with					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_8_2631_s_334	10436018	A Lys to Ala mutation within the highly conserved Walker A motif of GST-HsCdc6 strongly reduced ATP-binding activity, and GST alone did not bind to ATP (Figure  1), demonstrating that complex formation with ATP is an intrinsic function of HsCdc6.	bind
47972	2	10785	5	13	NULL	NULL	NULL	GST-HsCdc6	GP		bind					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_8_2631_s_334	10436018	A Lys to Ala mutation within the highly conserved Walker A motif of GST-HsCdc6 strongly reduced ATP-binding activity, and GST alone did not bind to ATP (Figure  1), demonstrating that complex formation with ATP is an intrinsic function of HsCdc6.	bind
47973	3	10785	5	13	NULL	NULL	NULL	GST-HsCdc6	GP		is mutated to			Lys in Walker A motif		GST-HsCdc6	GP		Ala in Walker A motif		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_8_2631_s_334	10436018	A Lys to Ala mutation within the highly conserved Walker A motif of GST-HsCdc6 strongly reduced ATP-binding activity, and GST alone did not bind to ATP (Figure  1), demonstrating that complex formation with ATP is an intrinsic function of HsCdc6.	bind
47974	4	10785	5	13	NULL	NULL	NULL	statement 3	Process		reduces		strongly			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_8_2631_s_334	10436018	A Lys to Ala mutation within the highly conserved Walker A motif of GST-HsCdc6 strongly reduced ATP-binding activity, and GST alone did not bind to ATP (Figure  1), demonstrating that complex formation with ATP is an intrinsic function of HsCdc6.	bind
47975	5	10785	5	13	NULL	NULL	NULL	GST	GP		does not bind					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_8_2631_s_334	10436018	A Lys to Ala mutation within the highly conserved Walker A motif of GST-HsCdc6 strongly reduced ATP-binding activity, and GST alone did not bind to ATP (Figure  1), demonstrating that complex formation with ATP is an intrinsic function of HsCdc6.	bind
47189	1	10785	6	NULL	NULL	0	NULL	GST-HsCdc6	NULL		is mutated to	NULL		Lys;; Walker A motif		GST-HsCdc6	NULL		Ala;; Walker A motif		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_10_8_2631_s_334	10436018	A Lys to Ala mutation within the highly conserved Walker A motif of GST-HsCdc6 strongly reduced ATP-binding activity, and GST alone did not bind to ATP (Figure  1), demonstrating that complex formation with ATP is an intrinsic function of HsCdc6.	bind
47190	2	10785	6	NULL	NULL	0	NULL	GST-HsCdc6	NULL		bind	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_10_8_2631_s_334	10436018	A Lys to Ala mutation within the highly conserved Walker A motif of GST-HsCdc6 strongly reduced ATP-binding activity, and GST alone did not bind to ATP (Figure  1), demonstrating that complex formation with ATP is an intrinsic function of HsCdc6.	bind
47191	3	10785	6	NULL	NULL	0	NULL	statement 1	NULL		reduces	NULL	strongly			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_10_8_2631_s_334	10436018	A Lys to Ala mutation within the highly conserved Walker A motif of GST-HsCdc6 strongly reduced ATP-binding activity, and GST alone did not bind to ATP (Figure  1), demonstrating that complex formation with ATP is an intrinsic function of HsCdc6.	bind
47192	4	10785	6	NULL	NULL	0	NULL	GST	NULL		does not bind	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_10_8_2631_s_334	10436018	A Lys to Ala mutation within the highly conserved Walker A motif of GST-HsCdc6 strongly reduced ATP-binding activity, and GST alone did not bind to ATP (Figure  1), demonstrating that complex formation with ATP is an intrinsic function of HsCdc6.	bind
49689	1	10788	5	13	NULL	NULL	NULL	beta MHC	GP	human	is changed to			lysine at amino acid 184		beta MHC	GP	human	arginine at amino acid 184		NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-cell-biol_137_1_9105042_s_5	9105042	A lysine to arginine  change at amino acid 184 in the consensus ATP binding sequence of human  beta MHC resulted in abnormal subcellular localization and disrupted both  thick and thin filament structure in transfected NRC.	bind
49690	2	10788	5	13	NULL	NULL	NULL	statement 1	Process		results in					beta MHC	GP	abnormal;;subcellular localization of;;human			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-cell-biol_137_1_9105042_s_5	9105042	A lysine to arginine  change at amino acid 184 in the consensus ATP binding sequence of human  beta MHC resulted in abnormal subcellular localization and disrupted both  thick and thin filament structure in transfected NRC.	bind
49691	3	10788	5	13	NULL	NULL	NULL	statement 1	Process		disrupts					thin filament	GP	structure of			NULL	transfected NRC	NULL	NULL	NULL	NULL	abs-batch0720-0739_j-cell-biol_137_1_9105042_s_5	9105042	A lysine to arginine  change at amino acid 184 in the consensus ATP binding sequence of human  beta MHC resulted in abnormal subcellular localization and disrupted both  thick and thin filament structure in transfected NRC.	bind
49692	4	10788	5	13	NULL	NULL	NULL	statement 1	Process		disrupts					thick filament	GP	structure of			NULL	transfected NRC	NULL	NULL	NULL	NULL	abs-batch0720-0739_j-cell-biol_137_1_9105042_s_5	9105042	A lysine to arginine  change at amino acid 184 in the consensus ATP binding sequence of human  beta MHC resulted in abnormal subcellular localization and disrupted both  thick and thin filament structure in transfected NRC.	bind
47193	1	10788	6	NULL	NULL	0	NULL	beta MHC	NULL	human	is changed to	NULL		lysine ;; amino acid 184		beta MHC	NULL	human	arginine;; amino acid 184		NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-cell-biol_137_1_9105042_s_5	9105042	A lysine to arginine  change at amino acid 184 in the consensus ATP binding sequence of human  beta MHC resulted in abnormal subcellular localization and disrupted both  thick and thin filament structure in transfected NRC.	bind
47194	2	10788	6	NULL	NULL	0	NULL	statement 1	NULL		results in abnormal	NULL				beta MHC	NULL	human;; subcellular localization of 			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-cell-biol_137_1_9105042_s_5	9105042	A lysine to arginine  change at amino acid 184 in the consensus ATP binding sequence of human  beta MHC resulted in abnormal subcellular localization and disrupted both  thick and thin filament structure in transfected NRC.	bind
47195	3	10788	6	NULL	NULL	0	NULL	statement 1	NULL		disrupts	NULL				thick filament	NULL	structure of			NULL	transfected NRC	0	NULL	NULL	NULL	abs-batch0720-0739_j-cell-biol_137_1_9105042_s_5	9105042	A lysine to arginine  change at amino acid 184 in the consensus ATP binding sequence of human  beta MHC resulted in abnormal subcellular localization and disrupted both  thick and thin filament structure in transfected NRC.	bind
47196	4	10788	6	NULL	NULL	0	NULL	statement 1	NULL		disrupts	NULL				thin filament	NULL	structure of			NULL	transfected NRC	0	NULL	NULL	NULL	abs-batch0720-0739_j-cell-biol_137_1_9105042_s_5	9105042	A lysine to arginine  change at amino acid 184 in the consensus ATP binding sequence of human  beta MHC resulted in abnormal subcellular localization and disrupted both  thick and thin filament structure in transfected NRC.	bind
49693	1	10790	5	13	NULL	NULL	NULL	NT-3	GP		bind					p75 receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_21_22_8915_s_398	11698603	A lysosomal pathway of NT-3 may be common to all neurotrophins and may involve binding to the p75 receptor ( U) or binding of NT-3 to trkC receptor ( Y) in the presence of the tyrosine kinase inhibitor K252a.	bind
49694	2	10790	5	13	NULL	NULL	NULL	statement 1	Process		in the presence of					K252a	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_21_22_8915_s_398	11698603	A lysosomal pathway of NT-3 may be common to all neurotrophins and may involve binding to the p75 receptor ( U) or binding of NT-3 to trkC receptor ( Y) in the presence of the tyrosine kinase inhibitor K252a.	bind
49695	3	10790	5	13	NULL	NULL	NULL	K252a	Chemical		is a type of					tyrosine kinase inhibitor	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_21_22_8915_s_398	11698603	A lysosomal pathway of NT-3 may be common to all neurotrophins and may involve binding to the p75 receptor ( U) or binding of NT-3 to trkC receptor ( Y) in the presence of the tyrosine kinase inhibitor K252a.	bind
49696	4	10790	5	13	NULL	NULL	NULL	NT-3	GP		bind					trkC receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_21_22_8915_s_398	11698603	A lysosomal pathway of NT-3 may be common to all neurotrophins and may involve binding to the p75 receptor ( U) or binding of NT-3 to trkC receptor ( Y) in the presence of the tyrosine kinase inhibitor K252a.	bind
49697	5	10790	5	13	NULL	NULL	NULL	statement 4	Process		in the presence of					K252a	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_21_22_8915_s_398	11698603	A lysosomal pathway of NT-3 may be common to all neurotrophins and may involve binding to the p75 receptor ( U) or binding of NT-3 to trkC receptor ( Y) in the presence of the tyrosine kinase inhibitor K252a.	bind
49698	6	10790	5	13	NULL	NULL	NULL	lysosomal pathway of NT-3	Process		involves		may			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_21_22_8915_s_398	11698603	A lysosomal pathway of NT-3 may be common to all neurotrophins and may involve binding to the p75 receptor ( U) or binding of NT-3 to trkC receptor ( Y) in the presence of the tyrosine kinase inhibitor K252a.	bind
49699	7	10790	5	13	NULL	NULL	NULL	lysosomal pathway of NT-3	Process		involves		may			statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_21_22_8915_s_398	11698603	A lysosomal pathway of NT-3 may be common to all neurotrophins and may involve binding to the p75 receptor ( U) or binding of NT-3 to trkC receptor ( Y) in the presence of the tyrosine kinase inhibitor K252a.	bind
49700	8	10790	5	13	NULL	NULL	NULL	lysosomal pathway of NT-3	Process		is common to					neurotrophins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_21_22_8915_s_398	11698603	A lysosomal pathway of NT-3 may be common to all neurotrophins and may involve binding to the p75 receptor ( U) or binding of NT-3 to trkC receptor ( Y) in the presence of the tyrosine kinase inhibitor K252a.	bind
47197	1	10790	6	10	NULL	0	NULL	NT-3	NULL		bind	NULL				p75 receptor	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_21_22_8915_s_398	11698603	A lysosomal pathway of NT-3 may be common to all neurotrophins and may involve binding to the p75 receptor ( U) or binding of NT-3 to trkC receptor ( Y) in the presence of the tyrosine kinase inhibitor K252a.	bind
47198	2	10790	6	10	NULL	0	NULL	NT-3	NULL		bind	NULL				trkC receptor	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_21_22_8915_s_398	11698603	A lysosomal pathway of NT-3 may be common to all neurotrophins and may involve binding to the p75 receptor ( U) or binding of NT-3 to trkC receptor ( Y) in the presence of the tyrosine kinase inhibitor K252a.	bind
47199	3	10790	6	NULL	NULL	0	NULL	lysosomal pathway of NT-3	NULL		is common to	NULL	may			neurotrophins	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_22_8915_s_398	11698603	A lysosomal pathway of NT-3 may be common to all neurotrophins and may involve binding to the p75 receptor ( U) or binding of NT-3 to trkC receptor ( Y) in the presence of the tyrosine kinase inhibitor K252a.	bind
47200	4	10790	6	NULL	NULL	0	NULL	statement 3	NULL		involve	NULL	may			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_22_8915_s_398	11698603	A lysosomal pathway of NT-3 may be common to all neurotrophins and may involve binding to the p75 receptor ( U) or binding of NT-3 to trkC receptor ( Y) in the presence of the tyrosine kinase inhibitor K252a.	bind
47201	5	10790	6	NULL	NULL	0	NULL	statement 3	NULL		involve	NULL	may			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_22_8915_s_398	11698603	A lysosomal pathway of NT-3 may be common to all neurotrophins and may involve binding to the p75 receptor ( U) or binding of NT-3 to trkC receptor ( Y) in the presence of the tyrosine kinase inhibitor K252a.	bind
47202	6	10790	6	NULL	NULL	0	NULL	statement 1	NULL		occurs in presence of	NULL				K252a	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_22_8915_s_398	11698603	A lysosomal pathway of NT-3 may be common to all neurotrophins and may involve binding to the p75 receptor ( U) or binding of NT-3 to trkC receptor ( Y) in the presence of the tyrosine kinase inhibitor K252a.	bind
47203	7	10790	6	NULL	NULL	0	NULL	statement 2	NULL		occurs in presence of	NULL				K252a	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_22_8915_s_398	11698603	A lysosomal pathway of NT-3 may be common to all neurotrophins and may involve binding to the p75 receptor ( U) or binding of NT-3 to trkC receptor ( Y) in the presence of the tyrosine kinase inhibitor K252a.	bind
47204	8	10790	6	NULL	NULL	0	NULL	K252a	NULL		is a type of	NULL				tyrosine kinase inhibitor	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_22_8915_s_398	11698603	A lysosomal pathway of NT-3 may be common to all neurotrophins and may involve binding to the p75 receptor ( U) or binding of NT-3 to trkC receptor ( Y) in the presence of the tyrosine kinase inhibitor K252a.	bind
49701	1	10791	5	13	NULL	NULL	NULL	TRA-2-10, IgG1	GP		is a type of					mAb against 2102ep	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_fertil-steril_58_3_1521662_s_2	1521662	A mAb (TRA-2-10, IgG1) to an embryonal carcinoma cell line (2102ep) that  recognizes an antigen termed membrane cofactor protein (CD 46, TLX antigen)  binds to human sperm after chemical induction of acrosomal loss by Ca2+  ionophore.	bind
49702	2	10791	5	13	NULL	NULL	NULL	2102ep	Cell		is a type of					embryonal carcinoma cell line	Cell				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_fertil-steril_58_3_1521662_s_2	1521662	A mAb (TRA-2-10, IgG1) to an embryonal carcinoma cell line (2102ep) that  recognizes an antigen termed membrane cofactor protein (CD 46, TLX antigen)  binds to human sperm after chemical induction of acrosomal loss by Ca2+  ionophore.	bind
49703	3	10791	5	13	NULL	NULL	NULL	CD 46	GP		is a type of					antigen	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_fertil-steril_58_3_1521662_s_2	1521662	A mAb (TRA-2-10, IgG1) to an embryonal carcinoma cell line (2102ep) that  recognizes an antigen termed membrane cofactor protein (CD 46, TLX antigen)  binds to human sperm after chemical induction of acrosomal loss by Ca2+  ionophore.	bind
49704	4	10791	5	13	NULL	NULL	NULL	CD 46	GP		is a type of					membrane cofactor protein	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_fertil-steril_58_3_1521662_s_2	1521662	A mAb (TRA-2-10, IgG1) to an embryonal carcinoma cell line (2102ep) that  recognizes an antigen termed membrane cofactor protein (CD 46, TLX antigen)  binds to human sperm after chemical induction of acrosomal loss by Ca2+  ionophore.	bind
49705	5	10791	5	13	NULL	NULL	NULL	TRA-2-10, IgG1	GP		bind					sperm	Cell	human			NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_fertil-steril_58_3_1521662_s_2	1521662	A mAb (TRA-2-10, IgG1) to an embryonal carcinoma cell line (2102ep) that  recognizes an antigen termed membrane cofactor protein (CD 46, TLX antigen)  binds to human sperm after chemical induction of acrosomal loss by Ca2+  ionophore.	bind
49706	6	10791	5	13	NULL	NULL	NULL	Ca2+ ionophore	Chemical		induce		chemically			acrosome	CellComponent	loss of			NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_fertil-steril_58_3_1521662_s_2	1521662	A mAb (TRA-2-10, IgG1) to an embryonal carcinoma cell line (2102ep) that  recognizes an antigen termed membrane cofactor protein (CD 46, TLX antigen)  binds to human sperm after chemical induction of acrosomal loss by Ca2+  ionophore.	bind
49707	7	10791	5	13	NULL	NULL	NULL	statement 5	Process		occurs after					statement 6	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_fertil-steril_58_3_1521662_s_2	1521662	A mAb (TRA-2-10, IgG1) to an embryonal carcinoma cell line (2102ep) that  recognizes an antigen termed membrane cofactor protein (CD 46, TLX antigen)  binds to human sperm after chemical induction of acrosomal loss by Ca2+  ionophore.	bind
50812	8	10791	5	13	NULL	NULL	NULL	TLX antigen	GP		is a type of					antigen	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_fertil-steril_58_3_1521662_s_2	1521662	A mAb (TRA-2-10, IgG1) to an embryonal carcinoma cell line (2102ep) that  recognizes an antigen termed membrane cofactor protein (CD 46, TLX antigen)  binds to human sperm after chemical induction of acrosomal loss by Ca2+  ionophore.	bind
50813	9	10791	5	13	NULL	NULL	NULL	TLX antigen	GP		is a type of					membrane cofactor protein \t	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_fertil-steril_58_3_1521662_s_2	1521662	A mAb (TRA-2-10, IgG1) to an embryonal carcinoma cell line (2102ep) that  recognizes an antigen termed membrane cofactor protein (CD 46, TLX antigen)  binds to human sperm after chemical induction of acrosomal loss by Ca2+  ionophore.	bind
47352	1	10791	6	10	NULL	0	NULL	CD46 	NULL		is a type of	NULL				membrane cofactor protein	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_fertil-steril_58_3_1521662_s_2	1521662	A mAb (TRA-2-10, IgG1) to an embryonal carcinoma cell line (2102ep) that  recognizes an antigen termed membrane cofactor protein (CD 46, TLX antigen)  binds to human sperm after chemical induction of acrosomal loss by Ca2+  ionophore.	bind
47353	2	10791	6	10	NULL	0	NULL	TLX antigen 	NULL		is a type of	NULL				membrane cofactor protein	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_fertil-steril_58_3_1521662_s_2	1521662	A mAb (TRA-2-10, IgG1) to an embryonal carcinoma cell line (2102ep) that  recognizes an antigen termed membrane cofactor protein (CD 46, TLX antigen)  binds to human sperm after chemical induction of acrosomal loss by Ca2+  ionophore.	bind
47354	3	10791	6	NULL	NULL	0	NULL	CD 46	NULL		is a type of	NULL				antigen	NULL				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_fertil-steril_58_3_1521662_s_2	1521662	A mAb (TRA-2-10, IgG1) to an embryonal carcinoma cell line (2102ep) that  recognizes an antigen termed membrane cofactor protein (CD 46, TLX antigen)  binds to human sperm after chemical induction of acrosomal loss by Ca2+  ionophore.	bind
47355	4	10791	6	NULL	NULL	0	NULL	TLX antigen	NULL		is a type of	NULL				antigen	NULL				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_fertil-steril_58_3_1521662_s_2	1521662	A mAb (TRA-2-10, IgG1) to an embryonal carcinoma cell line (2102ep) that  recognizes an antigen termed membrane cofactor protein (CD 46, TLX antigen)  binds to human sperm after chemical induction of acrosomal loss by Ca2+  ionophore.	bind
47356	5	10791	6	NULL	NULL	0	NULL	TRA-2-10, IgG1	NULL		is a type of	NULL				mAb against 2101ep	NULL				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_fertil-steril_58_3_1521662_s_2	1521662	A mAb (TRA-2-10, IgG1) to an embryonal carcinoma cell line (2102ep) that  recognizes an antigen termed membrane cofactor protein (CD 46, TLX antigen)  binds to human sperm after chemical induction of acrosomal loss by Ca2+  ionophore.	bind
47357	6	10791	6	NULL	NULL	0	NULL	2102ep	NULL		is a type of	NULL				embryonal carcinoma cell line	NULL				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_fertil-steril_58_3_1521662_s_2	1521662	A mAb (TRA-2-10, IgG1) to an embryonal carcinoma cell line (2102ep) that  recognizes an antigen termed membrane cofactor protein (CD 46, TLX antigen)  binds to human sperm after chemical induction of acrosomal loss by Ca2+  ionophore.	bind
47362	7	10791	6	NULL	NULL	0	NULL	TRA-2-10, IgG1	NULL		bind	NULL				sperm	NULL	human			NULL		0	NULL	NULL	NULL	abs-batch0680-0699_fertil-steril_58_3_1521662_s_2	1521662	A mAb (TRA-2-10, IgG1) to an embryonal carcinoma cell line (2102ep) that  recognizes an antigen termed membrane cofactor protein (CD 46, TLX antigen)  binds to human sperm after chemical induction of acrosomal loss by Ca2+  ionophore.	bind
47363	8	10791	6	10	NULL	0	NULL	Ca2+ ionophore	NULL		induces	NULL				acrosome	NULL	loss of			NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_fertil-steril_58_3_1521662_s_2	1521662	A mAb (TRA-2-10, IgG1) to an embryonal carcinoma cell line (2102ep) that  recognizes an antigen termed membrane cofactor protein (CD 46, TLX antigen)  binds to human sperm after chemical induction of acrosomal loss by Ca2+  ionophore.	bind
47364	9	10791	6	NULL	NULL	0	NULL	statement 7	NULL		occurs after	NULL				statement 8	NULL				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_fertil-steril_58_3_1521662_s_2	1521662	A mAb (TRA-2-10, IgG1) to an embryonal carcinoma cell line (2102ep) that  recognizes an antigen termed membrane cofactor protein (CD 46, TLX antigen)  binds to human sperm after chemical induction of acrosomal loss by Ca2+  ionophore.	bind
49708	1	10792	5	13	NULL	NULL	NULL	mAb against an alpha spectrin	GP		bind					230-kDa protein	GP				NULL	HeLa chromatin-associated protein extracts	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_46_32904_s_85	10551855	A mAb against an alpha spectrin, with specificity for mammalian nonerythroid alpha spectrin (Chemicon), bound to the 230-kDa protein from HeLa chromatin-associated protein extracts (Fig.  1,  lane 1); binding of this mAb to human erythroid spectrin (alpha and beta chains) (Fig.  1,  lane 2) was used as a control.	bind
49709	2	10792	5	13	NULL	NULL	NULL	mAb against an alpha spectrin	GP		is specific to					nonerythroid alpha spectrin	GP	mammalian			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_46_32904_s_85	10551855	A mAb against an alpha spectrin, with specificity for mammalian nonerythroid alpha spectrin (Chemicon), bound to the 230-kDa protein from HeLa chromatin-associated protein extracts (Fig.  1,  lane 1); binding of this mAb to human erythroid spectrin (alpha and beta chains) (Fig.  1,  lane 2) was used as a control.	bind
49710	3	10792	5	13	NULL	NULL	NULL	mAb against an alpha spectrin	GP		bind					erythroid spectrin	GP	human	alpha chain;;beta chain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_46_32904_s_85	10551855	A mAb against an alpha spectrin, with specificity for mammalian nonerythroid alpha spectrin (Chemicon), bound to the 230-kDa protein from HeLa chromatin-associated protein extracts (Fig.  1,  lane 1); binding of this mAb to human erythroid spectrin (alpha and beta chains) (Fig.  1,  lane 2) was used as a control.	bind
47365	1	10792	6	NULL	NULL	0	NULL	230-kDa protein	NULL		isolated from	NULL				HeLa chromatin-associated protein extracts	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_46_32904_s_85	10551855	A mAb against an alpha spectrin, with specificity for mammalian nonerythroid alpha spectrin (Chemicon), bound to the 230-kDa protein from HeLa chromatin-associated protein extracts (Fig.  1,  lane 1); binding of this mAb to human erythroid spectrin (alpha and beta chains) (Fig.  1,  lane 2) was used as a control.	bind
47366	2	10792	6	NULL	NULL	0	NULL	mAb against an alpha spectrin	NULL		bind	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_46_32904_s_85	10551855	A mAb against an alpha spectrin, with specificity for mammalian nonerythroid alpha spectrin (Chemicon), bound to the 230-kDa protein from HeLa chromatin-associated protein extracts (Fig.  1,  lane 1); binding of this mAb to human erythroid spectrin (alpha and beta chains) (Fig.  1,  lane 2) was used as a control.	bind
47367	3	10792	6	NULL	NULL	0	NULL	mAb against alpha spectrin	NULL		bind	NULL				erythroid spectrin	NULL	human	alpha chain;; beta chain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_46_32904_s_85	10551855	A mAb against an alpha spectrin, with specificity for mammalian nonerythroid alpha spectrin (Chemicon), bound to the 230-kDa protein from HeLa chromatin-associated protein extracts (Fig.  1,  lane 1); binding of this mAb to human erythroid spectrin (alpha and beta chains) (Fig.  1,  lane 2) was used as a control.	bind
50374	4	10792	6	10	NULL	0	NULL	mAb against alpha spectrin	NULL		is specific to	NULL				nonerythroid alpha spectrin	NULL	mammalian			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_46_32904_s_85	10551855	A mAb against an alpha spectrin, with specificity for mammalian nonerythroid alpha spectrin (Chemicon), bound to the 230-kDa protein from HeLa chromatin-associated protein extracts (Fig.  1,  lane 1); binding of this mAb to human erythroid spectrin (alpha and beta chains) (Fig.  1,  lane 2) was used as a control.	bind
49711	1	10793	5	13	NULL	NULL	NULL	Fn	GP		bind			HBD		M. tuberculosis	Organism				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_3_1287_s_161	11854212	A MAb specific to the HBD of Fn, but not to the CBD or GBD of Fn, decreased binding of Fn to  M. tuberculosis, suggesting that the HBD is the site on the Fn molecule responsible for Fn binding to  M. tuberculosis.	bind
47368	1	10793	6	NULL	NULL	0	NULL	Fn	NULL		bind	NULL		HBD		M. tuberculosis	NULL				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_3_1287_s_161	11854212	A MAb specific to the HBD of Fn, but not to the CBD or GBD of Fn, decreased binding of Fn to  M. tuberculosis, suggesting that the HBD is the site on the Fn molecule responsible for Fn binding to  M. tuberculosis.	bind
49712	2	10795	5	13	NULL	NULL	NULL	MAGP-1	GP		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_22_23045_s_233	15044481	A MAGP-1-binding site in exon 1 would be compatible with the studies of Jensen  et al. ( ), who showed positive MAGP-1 binding to a fibrillin-1 fragment encoding exons 1 - 11 but negative binding to fragments spanning this region but lacking exons 1 - 3.	bind
49713	3	10795	5	13	NULL	NULL	NULL	MAGP-1	GP		does not bind					fibrillin-1 fragment	GP	lacking		exons 1 - 3	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_22_23045_s_233	15044481	A MAGP-1-binding site in exon 1 would be compatible with the studies of Jensen  et al. ( ), who showed positive MAGP-1 binding to a fibrillin-1 fragment encoding exons 1 - 11 but negative binding to fragments spanning this region but lacking exons 1 - 3.	bind
50375	1	10795	5	13	NULL	NULL	NULL	 fibrillin-1 fragment 	GP		encode									exons 1-11	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_22_23045_s_233	15044481	A MAGP-1-binding site in exon 1 would be compatible with the studies of Jensen  et al. ( ), who showed positive MAGP-1 binding to a fibrillin-1 fragment encoding exons 1 - 11 but negative binding to fragments spanning this region but lacking exons 1 - 3.	bind
47219	1	10795	6	10	NULL	0	NULL	fibrillin-1 fragment	NULL		encodes	NULL					NULL			exons 1-11	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_22_23045_s_233	15044481	A MAGP-1-binding site in exon 1 would be compatible with the studies of Jensen  et al. ( ), who showed positive MAGP-1 binding to a fibrillin-1 fragment encoding exons 1 - 11 but negative binding to fragments spanning this region but lacking exons 1 - 3.	bind
47221	2	10795	6	NULL	NULL	0	NULL	MAGP-1 	NULL		bind	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_22_23045_s_233	15044481	A MAGP-1-binding site in exon 1 would be compatible with the studies of Jensen  et al. ( ), who showed positive MAGP-1 binding to a fibrillin-1 fragment encoding exons 1 - 11 but negative binding to fragments spanning this region but lacking exons 1 - 3.	bind
47226	3	10795	6	NULL	NULL	0	NULL	MAGP-1	NULL		does not bind	NULL				fibrillin-1 fragment 	NULL	lacking		exons 1-3	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_22_23045_s_233	15044481	A MAGP-1-binding site in exon 1 would be compatible with the studies of Jensen  et al. ( ), who showed positive MAGP-1 binding to a fibrillin-1 fragment encoding exons 1 - 11 but negative binding to fragments spanning this region but lacking exons 1 - 3.	bind
49714	1	10796	5	13	NULL	NULL	NULL	PCNA	GP		bind					RF-C	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_3_1769_s_203	8999859	A main goal of this work was to begin characterizing the molecular interactions between RF-C and PCNA by first determining the region within PCNA that is bound by RF-C.	bind
47231	1	10796	6	NULL	NULL	0	NULL	PCNA	NULL		bind	NULL				RF-C	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_3_1769_s_203	8999859	A main goal of this work was to begin characterizing the molecular interactions between RF-C and PCNA by first determining the region within PCNA that is bound by RF-C.	bind
49715	1	10797	5	13	NULL	NULL	NULL	zinc finger protein	GP	maize	bind					zein gene	GP			prolamin box in promoter	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_1_28_s_291	10640273	A maize zinc finger protein binds the prolamin box in zein gene promoters and interacts with basic leucine zipper transcriptional activator Opaque2.	bind
49716	2	10797	5	13	NULL	NULL	NULL	zinc finger protein	GP	maize	interacts with					Opaque2	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_1_28_s_291	10640273	A maize zinc finger protein binds the prolamin box in zein gene promoters and interacts with basic leucine zipper transcriptional activator Opaque2.	bind
49717	3	10797	5	13	NULL	NULL	NULL	Opaque2	GP		is a type of					basic leucine zipper transcriptional activator	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_1_28_s_291	10640273	A maize zinc finger protein binds the prolamin box in zein gene promoters and interacts with basic leucine zipper transcriptional activator Opaque2.	bind
47237	1	10797	6	10	NULL	0	NULL	zinc finger protein	NULL	maize	bind	NULL				zein gene	NULL			prolamin box of promoter	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_1_28_s_291	10640273	A maize zinc finger protein binds the prolamin box in zein gene promoters and interacts with basic leucine zipper transcriptional activator Opaque2.	bind
47238	2	10797	6	NULL	NULL	0	NULL	zinc finger protein	NULL	maize	interacts with	NULL				Opaque2	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_14_1_28_s_291	10640273	A maize zinc finger protein binds the prolamin box in zein gene promoters and interacts with basic leucine zipper transcriptional activator Opaque2.	bind
47240	3	10797	6	NULL	NULL	0	NULL	opaque 2	NULL		is a type of	NULL				basic leucine zipper transcriptional activator	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_14_1_28_s_291	10640273	A maize zinc finger protein binds the prolamin box in zein gene promoters and interacts with basic leucine zipper transcriptional activator Opaque2.	bind
49718	1	10800	5	13	NULL	NULL	NULL	HP1	GP		is					heterochromatin protein 1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_112_5_599_s_31	12628181	A major advance came from the discovery that mammalian heterochromatin protein 1 (HP1) binds methylated histone H3 tails  (Bannister et al., 2001  ).	bind
49719	2	10800	5	13	NULL	NULL	NULL	HP1	GP	mammalian	bind					histone H3 tails	GP	methylated			NULL		NULL	NULL	NULL	NULL	gw60_cell_112_5_599_s_31	12628181	A major advance came from the discovery that mammalian heterochromatin protein 1 (HP1) binds methylated histone H3 tails  (Bannister et al., 2001  ).	bind
47243	1	10800	6	NULL	NULL	0	NULL	HP1	NULL	mammalian	bind	NULL				Histone H3 tail	NULL	methylated			NULL		0	NULL	NULL	NULL	gw60_cell_112_5_599_s_31	12628181	A major advance came from the discovery that mammalian heterochromatin protein 1 (HP1) binds methylated histone H3 tails  (Bannister et al., 2001  ).	bind
47245	2	10800	6	NULL	NULL	0	NULL	HP1	NULL		is	NULL				heterochromatin protein 1	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_112_5_599_s_31	12628181	A major advance came from the discovery that mammalian heterochromatin protein 1 (HP1) binds methylated histone H3 tails  (Bannister et al., 2001  ).	bind
49720	1	10801	5	13	NULL	NULL	NULL	CBF3	GP		is a type of					multi subunit complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_30_0_7_s_203	8982447	A major advance in centromere research was the biochemical identification of CBF3,  a multi subunit complex that specifically binds CDEIII DNA ( 63).	bind
49721	2	10801	5	13	NULL	NULL	NULL	CBF3	GP		bind		specifically			CDEIII DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_30_0_7_s_203	8982447	A major advance in centromere research was the biochemical identification of CBF3,  a multi subunit complex that specifically binds CDEIII DNA ( 63).	bind
37944	1	10801	6	10	NULL	0	NULL	CBF3	NULL		is a type of	NULL				multi subunit complex	NULL				NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_30_0_7_s_203	8982447	A major advance in centromere research was the biochemical identification of CBF3,  a multi subunit complex that specifically binds CDEIII DNA ( 63).	bind
37945	2	10801	6	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL	specifically			CDEIII DNA	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevgenet_30_0_7_s_203	8982447	A major advance in centromere research was the biochemical identification of CBF3,  a multi subunit complex that specifically binds CDEIII DNA ( 63).	bind
49722	1	10802	5	13	NULL	NULL	NULL	CaBP1	GP		bind					alpha11.2	GP		NT		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_33_29612_s_216	15980432	A major assumption is that CaBP1 is constitutively associated with the channel via the NT of alpha11.2, which is based on our findings that CaBP1 binds to the NT in the presence and absence of Ca2+ ( Fig. 3).	bind
49723	2	10802	5	13	NULL	NULL	NULL	CaBP1	GP		is associated with		may;;constitutively			channel	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_33_29612_s_216	15980432	A major assumption is that CaBP1 is constitutively associated with the channel via the NT of alpha11.2, which is based on our findings that CaBP1 binds to the NT in the presence and absence of Ca2+ ( Fig. 3).	bind
49724	3	10802	5	13	NULL	NULL	NULL	statement 2	Process		via					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_33_29612_s_216	15980432	A major assumption is that CaBP1 is constitutively associated with the channel via the NT of alpha11.2, which is based on our findings that CaBP1 binds to the NT in the presence and absence of Ca2+ ( Fig. 3).	bind
37946	1	10802	6	10	NULL	0	NULL	CaBP1	NULL		bind	NULL				alpha11.2	NULL		NT		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_33_29612_s_216	15980432	A major assumption is that CaBP1 is constitutively associated with the channel via the NT of alpha11.2, which is based on our findings that CaBP1 binds to the NT in the presence and absence of Ca2+ ( Fig. 3).	bind
40507	2	10802	6	NULL	NULL	0	NULL	CaBP1	NULL		associated with	NULL	may be;; constitutively			channel	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_33_29612_s_216	15980432	A major assumption is that CaBP1 is constitutively associated with the channel via the NT of alpha11.2, which is based on our findings that CaBP1 binds to the NT in the presence and absence of Ca2+ ( Fig. 3).	bind
40508	3	10802	6	NULL	NULL	0	NULL	statement 2	NULL		is because of	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_33_29612_s_216	15980432	A major assumption is that CaBP1 is constitutively associated with the channel via the NT of alpha11.2, which is based on our findings that CaBP1 binds to the NT in the presence and absence of Ca2+ ( Fig. 3).	bind
49725	1	10804	5	13	NULL	NULL	NULL	RhoGDI	GP		associate with		directly			Rho proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_18_12445_s_158	16517596	A major class of proteins that directly associates with Rho proteins in cells is termed RhoGDI, and its binding to Rho GTPases is via an interaction that is known to be prenylation-dependent ( ).	bind
49726	2	10804	5	13	NULL	NULL	NULL	RhoGDI	GP		bind					Rho GTPases	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_18_12445_s_158	16517596	A major class of proteins that directly associates with Rho proteins in cells is termed RhoGDI, and its binding to Rho GTPases is via an interaction that is known to be prenylation-dependent ( ).	bind
49727	3	10804	5	13	NULL	NULL	NULL	statement 2	Process		is dependent on					prenylation	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_18_12445_s_158	16517596	A major class of proteins that directly associates with Rho proteins in cells is termed RhoGDI, and its binding to Rho GTPases is via an interaction that is known to be prenylation-dependent ( ).	bind
40509	1	10804	6	NULL	NULL	0	NULL	RhoGDI	NULL		bind	NULL				RhoGTPase	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_18_12445_s_158	16517596	A major class of proteins that directly associates with Rho proteins in cells is termed RhoGDI, and its binding to Rho GTPases is via an interaction that is known to be prenylation-dependent ( ).	bind
40510	2	10804	6	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				prenylation	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_18_12445_s_158	16517596	A major class of proteins that directly associates with Rho proteins in cells is termed RhoGDI, and its binding to Rho GTPases is via an interaction that is known to be prenylation-dependent ( ).	bind
50376	3	10804	6	10	NULL	0	NULL	RhoGDI	NULL		associate with	NULL	directly			Rho protein	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_18_12445_s_158	16517596	A major class of proteins that directly associates with Rho proteins in cells is termed RhoGDI, and its binding to Rho GTPases is via an interaction that is known to be prenylation-dependent ( ).	bind
49728	1	10805	5	13	NULL	NULL	NULL	CmtR	GP		bind					35-bp DNA fragment	NucleicAcid			degenerate 10 - 5-10 hyphenated-inverted repeat	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_45_44560_s_99	12939264	A major complex was detected with P2 and P3 but not with P4 ( Fig. 1 D), confirming CmtR binding to sequences contained within a 35-bp DNA fragment that includes a degenerate 10 - 5-10 hyphenated-inverted repeat ( Fig. 1 E).	bind
40193	1	10805	6	NULL	NULL	0	NULL	CmtR	NULL		bind	NULL				35-bp DNA	NULL			hyphenated-inverted repeat	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_45_44560_s_99	12939264	A major complex was detected with P2 and P3 but not with P4 ( Fig. 1 D), confirming CmtR binding to sequences contained within a 35-bp DNA fragment that includes a degenerate 10 - 5-10 hyphenated-inverted repeat ( Fig. 1 E).	bind
50792	1	10806	5	13	NULL	NULL	NULL	Ras	GP		induce					ARF	GP				NULL		NULL	NULL	NULL	NULL	gw60_cancercell_1_1_19_s_63	12086884	A major component of the differential that couples the oppositely spinning wheels of proliferation and growth suppression is the ARF/Mdm-2/p53 tumor suppressor pathway ( Sherr, 2001  ); Ras, E1A, Myc, and E2F all induce ARF, an alternate product of the  INK4a locus which then binds and inactivates Mdm-2, a key part of the ubiquitin ligase that keeps p53 at bay ( Lowe, 1999  ).	bind
50793	2	10806	5	13	NULL	NULL	NULL	E1A	GP		induce					ARF	GP				NULL		NULL	NULL	NULL	NULL	gw60_cancercell_1_1_19_s_63	12086884	A major component of the differential that couples the oppositely spinning wheels of proliferation and growth suppression is the ARF/Mdm-2/p53 tumor suppressor pathway ( Sherr, 2001  ); Ras, E1A, Myc, and E2F all induce ARF, an alternate product of the  INK4a locus which then binds and inactivates Mdm-2, a key part of the ubiquitin ligase that keeps p53 at bay ( Lowe, 1999  ).	bind
50794	3	10806	5	13	NULL	NULL	NULL	Myc	GP		induce					ARF	GP				NULL		NULL	NULL	NULL	NULL	gw60_cancercell_1_1_19_s_63	12086884	A major component of the differential that couples the oppositely spinning wheels of proliferation and growth suppression is the ARF/Mdm-2/p53 tumor suppressor pathway ( Sherr, 2001  ); Ras, E1A, Myc, and E2F all induce ARF, an alternate product of the  INK4a locus which then binds and inactivates Mdm-2, a key part of the ubiquitin ligase that keeps p53 at bay ( Lowe, 1999  ).	bind
50795	4	10806	5	13	NULL	NULL	NULL	E2F 	GP		induce					ARF	GP				NULL		NULL	NULL	NULL	NULL	gw60_cancercell_1_1_19_s_63	12086884	A major component of the differential that couples the oppositely spinning wheels of proliferation and growth suppression is the ARF/Mdm-2/p53 tumor suppressor pathway ( Sherr, 2001  ); Ras, E1A, Myc, and E2F all induce ARF, an alternate product of the  INK4a locus which then binds and inactivates Mdm-2, a key part of the ubiquitin ligase that keeps p53 at bay ( Lowe, 1999  ).	bind
50796	5	10806	5	13	NULL	NULL	NULL	ARF	GP		is an alternate product of					INK4a locus	GP				NULL		NULL	NULL	NULL	NULL	gw60_cancercell_1_1_19_s_63	12086884	A major component of the differential that couples the oppositely spinning wheels of proliferation and growth suppression is the ARF/Mdm-2/p53 tumor suppressor pathway ( Sherr, 2001  ); Ras, E1A, Myc, and E2F all induce ARF, an alternate product of the  INK4a locus which then binds and inactivates Mdm-2, a key part of the ubiquitin ligase that keeps p53 at bay ( Lowe, 1999  ).	bind
50797	6	10806	5	13	NULL	NULL	NULL	ARF	GP	induced	bind					Mdm-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cancercell_1_1_19_s_63	12086884	A major component of the differential that couples the oppositely spinning wheels of proliferation and growth suppression is the ARF/Mdm-2/p53 tumor suppressor pathway ( Sherr, 2001  ); Ras, E1A, Myc, and E2F all induce ARF, an alternate product of the  INK4a locus which then binds and inactivates Mdm-2, a key part of the ubiquitin ligase that keeps p53 at bay ( Lowe, 1999  ).	bind
50798	7	10806	5	13	NULL	NULL	NULL	statement 6	Process		inactivates					Mdm-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cancercell_1_1_19_s_63	12086884	A major component of the differential that couples the oppositely spinning wheels of proliferation and growth suppression is the ARF/Mdm-2/p53 tumor suppressor pathway ( Sherr, 2001  ); Ras, E1A, Myc, and E2F all induce ARF, an alternate product of the  INK4a locus which then binds and inactivates Mdm-2, a key part of the ubiquitin ligase that keeps p53 at bay ( Lowe, 1999  ).	bind
50799	8	10806	5	13	NULL	NULL	NULL	Mdm-2	GP		is a part of					ubiquitin ligase	GP				NULL		NULL	NULL	NULL	NULL	gw60_cancercell_1_1_19_s_63	12086884	A major component of the differential that couples the oppositely spinning wheels of proliferation and growth suppression is the ARF/Mdm-2/p53 tumor suppressor pathway ( Sherr, 2001  ); Ras, E1A, Myc, and E2F all induce ARF, an alternate product of the  INK4a locus which then binds and inactivates Mdm-2, a key part of the ubiquitin ligase that keeps p53 at bay ( Lowe, 1999  ).	bind
40511	1	10806	6	NULL	NULL	0	NULL	Ras	NULL		induce	NULL				ARF	NULL				NULL		0	NULL	NULL	NULL	gw60_cancercell_1_1_19_s_63	12086884	A major component of the differential that couples the oppositely spinning wheels of proliferation and growth suppression is the ARF/Mdm-2/p53 tumor suppressor pathway ( Sherr, 2001  ); Ras, E1A, Myc, and E2F all induce ARF, an alternate product of the  INK4a locus which then binds and inactivates Mdm-2, a key part of the ubiquitin ligase that keeps p53 at bay ( Lowe, 1999  ).	bind
40512	2	10806	6	NULL	NULL	0	NULL	E1A	NULL		induce	NULL				ARF	NULL				NULL		0	NULL	NULL	NULL	gw60_cancercell_1_1_19_s_63	12086884	A major component of the differential that couples the oppositely spinning wheels of proliferation and growth suppression is the ARF/Mdm-2/p53 tumor suppressor pathway ( Sherr, 2001  ); Ras, E1A, Myc, and E2F all induce ARF, an alternate product of the  INK4a locus which then binds and inactivates Mdm-2, a key part of the ubiquitin ligase that keeps p53 at bay ( Lowe, 1999  ).	bind
40513	3	10806	6	NULL	NULL	0	NULL	Myc	NULL		induce	NULL				ARF	NULL				NULL		0	NULL	NULL	NULL	gw60_cancercell_1_1_19_s_63	12086884	A major component of the differential that couples the oppositely spinning wheels of proliferation and growth suppression is the ARF/Mdm-2/p53 tumor suppressor pathway ( Sherr, 2001  ); Ras, E1A, Myc, and E2F all induce ARF, an alternate product of the  INK4a locus which then binds and inactivates Mdm-2, a key part of the ubiquitin ligase that keeps p53 at bay ( Lowe, 1999  ).	bind
40514	4	10806	6	NULL	NULL	0	NULL	E2F	NULL		induce	NULL				ARF	NULL				NULL		0	NULL	NULL	NULL	gw60_cancercell_1_1_19_s_63	12086884	A major component of the differential that couples the oppositely spinning wheels of proliferation and growth suppression is the ARF/Mdm-2/p53 tumor suppressor pathway ( Sherr, 2001  ); Ras, E1A, Myc, and E2F all induce ARF, an alternate product of the  INK4a locus which then binds and inactivates Mdm-2, a key part of the ubiquitin ligase that keeps p53 at bay ( Lowe, 1999  ).	bind
40515	5	10806	6	NULL	NULL	0	NULL	ARF	NULL		is an alternate product of	NULL				INK4a locus	NULL				NULL		0	NULL	NULL	NULL	gw60_cancercell_1_1_19_s_63	12086884	A major component of the differential that couples the oppositely spinning wheels of proliferation and growth suppression is the ARF/Mdm-2/p53 tumor suppressor pathway ( Sherr, 2001  ); Ras, E1A, Myc, and E2F all induce ARF, an alternate product of the  INK4a locus which then binds and inactivates Mdm-2, a key part of the ubiquitin ligase that keeps p53 at bay ( Lowe, 1999  ).	bind
40516	6	10806	6	NULL	NULL	0	NULL	ARF	NULL	induced	bind	NULL				Mdm-2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cancercell_1_1_19_s_63	12086884	A major component of the differential that couples the oppositely spinning wheels of proliferation and growth suppression is the ARF/Mdm-2/p53 tumor suppressor pathway ( Sherr, 2001  ); Ras, E1A, Myc, and E2F all induce ARF, an alternate product of the  INK4a locus which then binds and inactivates Mdm-2, a key part of the ubiquitin ligase that keeps p53 at bay ( Lowe, 1999  ).	bind
40517	7	10806	6	10	NULL	0	NULL	statement 6			inactivates					Mdm-2					NULL		NULL	NULL	NULL	NULL	gw60_cancercell_1_1_19_s_63	12086884	A major component of the differential that couples the oppositely spinning wheels of proliferation and growth suppression is the ARF/Mdm-2/p53 tumor suppressor pathway ( Sherr, 2001  ); Ras, E1A, Myc, and E2F all induce ARF, an alternate product of the  INK4a locus which then binds and inactivates Mdm-2, a key part of the ubiquitin ligase that keeps p53 at bay ( Lowe, 1999  ).	bind
40518	8	10806	6	NULL	NULL	0	NULL	Mdm-2	NULL		is a key part of	NULL				ubiquitin ligase	NULL				NULL		0	NULL	NULL	NULL	gw60_cancercell_1_1_19_s_63	12086884	A major component of the differential that couples the oppositely spinning wheels of proliferation and growth suppression is the ARF/Mdm-2/p53 tumor suppressor pathway ( Sherr, 2001  ); Ras, E1A, Myc, and E2F all induce ARF, an alternate product of the  INK4a locus which then binds and inactivates Mdm-2, a key part of the ubiquitin ligase that keeps p53 at bay ( Lowe, 1999  ).	bind
49729	1	10807	5	13	NULL	NULL	NULL	HDL	GP		bind					SR-BI	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochemistry_39_1_10625497_s_3	10625497	A major component of the enhanced FC flux appears to occur independently  of HDL binding to SR-BI and may be due to changes in membrane lipid domains  resulting from SR-BI expression (1).	bind
49730	2	10807	5	13	NULL	NULL	NULL	FC flux	Process	enhanced	is independent of					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochemistry_39_1_10625497_s_3	10625497	A major component of the enhanced FC flux appears to occur independently  of HDL binding to SR-BI and may be due to changes in membrane lipid domains  resulting from SR-BI expression (1).	bind
49731	3	10807	5	13	NULL	NULL	NULL	SR-BI	GP	expression of	results in					membrane lipid domains	GP	chnages in			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochemistry_39_1_10625497_s_3	10625497	A major component of the enhanced FC flux appears to occur independently  of HDL binding to SR-BI and may be due to changes in membrane lipid domains  resulting from SR-BI expression (1).	bind
49732	4	10807	5	13	NULL	NULL	NULL	FC flux	Process	enhanced	occurs due to		may			statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochemistry_39_1_10625497_s_3	10625497	A major component of the enhanced FC flux appears to occur independently  of HDL binding to SR-BI and may be due to changes in membrane lipid domains  resulting from SR-BI expression (1).	bind
40259	1	10807	6	NULL	NULL	0	NULL	HDL	NULL		bind	NULL				SR-BI	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_biochemistry_39_1_10625497_s_3	10625497	A major component of the enhanced FC flux appears to occur independently  of HDL binding to SR-BI and may be due to changes in membrane lipid domains  resulting from SR-BI expression (1).	bind
40266	2	10807	6	NULL	NULL	0	NULL	SR-BI	NULL	expression of	results in	NULL				membrane lipid domains	NULL	changes in			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_biochemistry_39_1_10625497_s_3	10625497	A major component of the enhanced FC flux appears to occur independently  of HDL binding to SR-BI and may be due to changes in membrane lipid domains  resulting from SR-BI expression (1).	bind
40267	3	10807	6	10	NULL	0	NULL	FC flux	NULL	enhanced	is due to	NULL	may			statement 2	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochemistry_39_1_10625497_s_3	10625497	A major component of the enhanced FC flux appears to occur independently  of HDL binding to SR-BI and may be due to changes in membrane lipid domains  resulting from SR-BI expression (1).	bind
40268	4	10807	6	NULL	NULL	0	NULL	FC flux	NULL		is independent of	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_biochemistry_39_1_10625497_s_3	10625497	A major component of the enhanced FC flux appears to occur independently  of HDL binding to SR-BI and may be due to changes in membrane lipid domains  resulting from SR-BI expression (1).	bind
49733	1	10808	5	13	NULL	NULL	NULL	MSH2	GP		is a component of		major			GT binding complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_46_36256_s_92	10954713	A major component of the GT binding complex is MSH2.	bind
40269	1	10808	6	10	NULL	0	NULL	MSH2			is a component of		major			GT binding complex					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_46_36256_s_92	10954713	A major component of the GT binding complex is MSH2.	bind
49734	1	10809	5	13	NULL	NULL	NULL	GDP	Chemical		bind					p21ras	GP				NULL		NULL	NULL	NULL	NULL	gw60_structure_4_4_475_s_312	8740369	A major conceptional constraint on any activation model is imposed by the observation that the GEF reduces the binding affinity of GDP and GTP to p21ras by a similar amount.	bind
49735	2	10809	5	13	NULL	NULL	NULL	GTP	Chemical		bind					p21ras	GP				NULL		NULL	NULL	NULL	NULL	gw60_structure_4_4_475_s_312	8740369	A major conceptional constraint on any activation model is imposed by the observation that the GEF reduces the binding affinity of GDP and GTP to p21ras by a similar amount.	bind
49736	3	10809	5	13	NULL	NULL	NULL	GEF	GP		reduces					statement 1	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_structure_4_4_475_s_312	8740369	A major conceptional constraint on any activation model is imposed by the observation that the GEF reduces the binding affinity of GDP and GTP to p21ras by a similar amount.	bind
49737	4	10809	5	13	NULL	NULL	NULL	GEF	GP		reduces					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_structure_4_4_475_s_312	8740369	A major conceptional constraint on any activation model is imposed by the observation that the GEF reduces the binding affinity of GDP and GTP to p21ras by a similar amount.	bind
40270	1	10809	6	NULL	NULL	0	NULL	GDP	NULL		bind	NULL				p21ras	NULL				NULL		0	NULL	NULL	NULL	gw60_structure_4_4_475_s_312	8740369	A major conceptional constraint on any activation model is imposed by the observation that the GEF reduces the binding affinity of GDP and GTP to p21ras by a similar amount.	bind
40271	2	10809	6	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				p21ras	NULL				NULL		0	NULL	NULL	NULL	gw60_structure_4_4_475_s_312	8740369	A major conceptional constraint on any activation model is imposed by the observation that the GEF reduces the binding affinity of GDP and GTP to p21ras by a similar amount.	bind
40272	3	10809	6	NULL	NULL	0	NULL	GEF	NULL		reduces	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_structure_4_4_475_s_312	8740369	A major conceptional constraint on any activation model is imposed by the observation that the GEF reduces the binding affinity of GDP and GTP to p21ras by a similar amount.	bind
40273	4	10809	6	NULL	NULL	0	NULL	GEF	NULL		reduces	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_structure_4_4_475_s_312	8740369	A major conceptional constraint on any activation model is imposed by the observation that the GEF reduces the binding affinity of GDP and GTP to p21ras by a similar amount.	bind
49765	1	10810	5	13	NULL	NULL	NULL	DnaA	NucleicAcid		bind									DnaA boxes	NULL	bacterial hosts	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_24_18454_s_30	10749858	A major difference between replication initiation in plasmid RK2 (as well as most of the DnaA-dependent plasmids studied so far) and that of chromosomal origins, is the fact that in most cases this plasmid requires, in addition to the binding of DnaA to DnaA boxes in most bacterial hosts, the binding of a plasmid encoded replication initiation protein to the origin for the formation of an open complex ( 16).	bind
49767	2	10810	5	13	NULL	NULL	NULL	replication initiation protein	NucleicAcid		bind					origin	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_24_18454_s_30	10749858	A major difference between replication initiation in plasmid RK2 (as well as most of the DnaA-dependent plasmids studied so far) and that of chromosomal origins, is the fact that in most cases this plasmid requires, in addition to the binding of DnaA to DnaA boxes in most bacterial hosts, the binding of a plasmid encoded replication initiation protein to the origin for the formation of an open complex ( 16).	bind
49768	3	10810	5	13	NULL	NULL	NULL	statement 2	Process		is required for					open complex	GP	formation of			NULL	plasmid RK2	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_24_18454_s_30	10749858	A major difference between replication initiation in plasmid RK2 (as well as most of the DnaA-dependent plasmids studied so far) and that of chromosomal origins, is the fact that in most cases this plasmid requires, in addition to the binding of DnaA to DnaA boxes in most bacterial hosts, the binding of a plasmid encoded replication initiation protein to the origin for the formation of an open complex ( 16).	bind
49769	4	10810	5	13	NULL	NULL	NULL	statement 1	Process		is required for					open complex	GP	formation of			NULL	plasmid RK2	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_24_18454_s_30	10749858	A major difference between replication initiation in plasmid RK2 (as well as most of the DnaA-dependent plasmids studied so far) and that of chromosomal origins, is the fact that in most cases this plasmid requires, in addition to the binding of DnaA to DnaA boxes in most bacterial hosts, the binding of a plasmid encoded replication initiation protein to the origin for the formation of an open complex ( 16).	bind
40519	1	10810	6	NULL	NULL	0	NULL	DnaA	NULL		bind	NULL					NULL			DnaA box	NULL	bacterial host	0	NULL	NULL	NULL	gw60_jbiolchem_275_24_18454_s_30	10749858	A major difference between replication initiation in plasmid RK2 (as well as most of the DnaA-dependent plasmids studied so far) and that of chromosomal origins, is the fact that in most cases this plasmid requires, in addition to the binding of DnaA to DnaA boxes in most bacterial hosts, the binding of a plasmid encoded replication initiation protein to the origin for the formation of an open complex ( 16).	bind
40520	2	10810	6	NULL	NULL	0	NULL	replication initiation protein	NULL		bind	NULL				origin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_24_18454_s_30	10749858	A major difference between replication initiation in plasmid RK2 (as well as most of the DnaA-dependent plasmids studied so far) and that of chromosomal origins, is the fact that in most cases this plasmid requires, in addition to the binding of DnaA to DnaA boxes in most bacterial hosts, the binding of a plasmid encoded replication initiation protein to the origin for the formation of an open complex ( 16).	bind
40521	3	10810	6	10	NULL	0	NULL	statement 2			is required for					open complex		formation of			NULL	plasmid RK2	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_24_18454_s_30	10749858	A major difference between replication initiation in plasmid RK2 (as well as most of the DnaA-dependent plasmids studied so far) and that of chromosomal origins, is the fact that in most cases this plasmid requires, in addition to the binding of DnaA to DnaA boxes in most bacterial hosts, the binding of a plasmid encoded replication initiation protein to the origin for the formation of an open complex ( 16).	bind
50377	4	10810	6	10	NULL	0	NULL	statement 1			is required for					open complex		formation of			NULL	plasmid RK2	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_24_18454_s_30	10749858	A major difference between replication initiation in plasmid RK2 (as well as most of the DnaA-dependent plasmids studied so far) and that of chromosomal origins, is the fact that in most cases this plasmid requires, in addition to the binding of DnaA to DnaA boxes in most bacterial hosts, the binding of a plasmid encoded replication initiation protein to the origin for the formation of an open complex ( 16).	bind
49770	1	10811	5	13	NULL	NULL	NULL	Ars/A1 BCR	GP		bind					autoantigen	GP	natural			NULL		NULL	NULL	NULL	NULL	gw60_immunity_14_1_33_s_205	11163228	A major difference between the Ars/A1 mouse and the HEL/anti-HEL model is the affinity of the anergy-inducing autoantigen: while the affinity of the receptor for HEL is  2 nanomolar ( Goodnow et al. 1988  ), several lines of evidence suggest that the Ars/A1 BCR binds its natural autoantigen with an affinity that is >10,000-fold lower.	bind
40274	1	10811	6	NULL	NULL	0	NULL	Ars/A1 BCR	NULL		bind	NULL				autoantigen	NULL	natural			NULL		0	NULL	NULL	NULL	gw60_immunity_14_1_33_s_205	11163228	A major difference between the Ars/A1 mouse and the HEL/anti-HEL model is the affinity of the anergy-inducing autoantigen: while the affinity of the receptor for HEL is  2 nanomolar ( Goodnow et al. 1988  ), several lines of evidence suggest that the Ars/A1 BCR binds its natural autoantigen with an affinity that is >10,000-fold lower.	bind
49771	1	10812	5	13	NULL	NULL	NULL	LC8	GP		interacts with					LC8 targets	GP		glutamine		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_23_21981_s_157	15701632	A major difference between the binding groove of LC8 and the putative TcTex-1 groove is at the site on LC8 that interacts with the invariant glutamine in LC8 targets ( Fig. 3,  B and  C).	bind
40522	1	10812	6	10	NULL	0	NULL	LC8			interacts with					LC8 targets			glutamine		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_23_21981_s_157	15701632	A major difference between the binding groove of LC8 and the putative TcTex-1 groove is at the site on LC8 that interacts with the invariant glutamine in LC8 targets ( Fig. 3,  B and  C).	bind
49772	1	10814	5	13	NULL	NULL	NULL	RA	Chemical		bind			carboxylate group		CRABP-II	GP	positively charged	 amino acid residues		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_9_4518_s_174	7876220	A major factor in the  binding of RA to CRABP-II involves the electrostatic interactions  between the carboxylate group of all- trans-RA and positively  charge amino acid residues in the protein( 9 ) .	bind
40285	1	10814	6	NULL	NULL	0	NULL	RA	NULL		bind	NULL		carboxylate group 		CRABP-II	NULL	positively charged	amino acids		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_9_4518_s_174	7876220	A major factor in the  binding of RA to CRABP-II involves the electrostatic interactions  between the carboxylate group of all- trans-RA and positively  charge amino acid residues in the protein( 9 ) .	bind
49773	1	10815	5	13	NULL	NULL	NULL	THP-1 macrophages	Cell		is stimulated by					LIGHT	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_14_2121_s_200	16186421	A major finding in the present study was the noticeable upregulation of SR-A in LIGHT-stimulated THP-1 macrophages, as shown at both the mRNA and protein level, as well as the increased binding of acLDL to this scavenger receptor.	bind
49774	2	10815	5	13	NULL	NULL	NULL	SR-A	GP		is upregulated in					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_14_2121_s_200	16186421	A major finding in the present study was the noticeable upregulation of SR-A in LIGHT-stimulated THP-1 macrophages, as shown at both the mRNA and protein level, as well as the increased binding of acLDL to this scavenger receptor.	bind
49775	3	10815	5	13	NULL	NULL	NULL	acLDL	GP		bind					SR-A	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_14_2121_s_200	16186421	A major finding in the present study was the noticeable upregulation of SR-A in LIGHT-stimulated THP-1 macrophages, as shown at both the mRNA and protein level, as well as the increased binding of acLDL to this scavenger receptor.	bind
49776	4	10815	5	13	NULL	NULL	NULL	SR-A	GP		is a type of					scavenger receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_14_2121_s_200	16186421	A major finding in the present study was the noticeable upregulation of SR-A in LIGHT-stimulated THP-1 macrophages, as shown at both the mRNA and protein level, as well as the increased binding of acLDL to this scavenger receptor.	bind
40289	1	10815	6	NULL	NULL	0	NULL	acLDL	NULL		bind	NULL				SR-A	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_14_2121_s_200	16186421	A major finding in the present study was the noticeable upregulation of SR-A in LIGHT-stimulated THP-1 macrophages, as shown at both the mRNA and protein level, as well as the increased binding of acLDL to this scavenger receptor.	bind
40290	2	10815	6	10	NULL	0	NULL	LIGHT	NULL		stimulate	NULL				THP-1 macrophages	NULL				NULL		NULL	NULL	NULL	NULL	gw70_circulation_112_14_2121_s_200	16186421	A major finding in the present study was the noticeable upregulation of SR-A in LIGHT-stimulated THP-1 macrophages, as shown at both the mRNA and protein level, as well as the increased binding of acLDL to this scavenger receptor.	bind
40291	3	10815	6	NULL	NULL	0	NULL	SR-A	NULL		is a type of	NULL				scavenger receptor	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_112_14_2121_s_200	16186421	A major finding in the present study was the noticeable upregulation of SR-A in LIGHT-stimulated THP-1 macrophages, as shown at both the mRNA and protein level, as well as the increased binding of acLDL to this scavenger receptor.	bind
50378	4	10815	6	10	NULL	0	NULL	SR-A	NULL		is upregulated in	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_circulation_112_14_2121_s_200	16186421	A major finding in the present study was the noticeable upregulation of SR-A in LIGHT-stimulated THP-1 macrophages, as shown at both the mRNA and protein level, as well as the increased binding of acLDL to this scavenger receptor.	bind
49777	1	10816	5	13	NULL	NULL	NULL	mechanical stretch	ResearchActivity		activates					p38 MAPK	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_23_24852_s_292	15051723	A major finding of the present study was that mechanical stretch activated p38 MAPK and that the activation of the kinase was necessary for wall stretch-induced GATA-4 binding to BNP promoter both in the left ventricle and in the atria.	bind
49778	2	10816	5	13	NULL	NULL	NULL	GATA-4	GP		is induced by					wall stretch	ResearchActivity				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_23_24852_s_292	15051723	A major finding of the present study was that mechanical stretch activated p38 MAPK and that the activation of the kinase was necessary for wall stretch-induced GATA-4 binding to BNP promoter both in the left ventricle and in the atria.	bind
49779	3	10816	5	13	NULL	NULL	NULL	statement 2	GP		bind					BNP	NucleicAcid			promoter	NULL	left ventricle	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_23_24852_s_292	15051723	A major finding of the present study was that mechanical stretch activated p38 MAPK and that the activation of the kinase was necessary for wall stretch-induced GATA-4 binding to BNP promoter both in the left ventricle and in the atria.	bind
49780	4	10816	5	13	NULL	NULL	NULL	statement 1	Process		is necessary for					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_23_24852_s_292	15051723	A major finding of the present study was that mechanical stretch activated p38 MAPK and that the activation of the kinase was necessary for wall stretch-induced GATA-4 binding to BNP promoter both in the left ventricle and in the atria.	bind
50379	5	10816	5	13	NULL	NULL	NULL	statement 2	GP		bind					BNP	NucleicAcid			promoter	NULL	atria	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_23_24852_s_292	15051723	A major finding of the present study was that mechanical stretch activated p38 MAPK and that the activation of the kinase was necessary for wall stretch-induced GATA-4 binding to BNP promoter both in the left ventricle and in the atria.	bind
50380	6	10816	5	13	NULL	NULL	NULL	statement 1	Process		is necessary for					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_23_24852_s_292	15051723	A major finding of the present study was that mechanical stretch activated p38 MAPK and that the activation of the kinase was necessary for wall stretch-induced GATA-4 binding to BNP promoter both in the left ventricle and in the atria.	bind
40292	1	10816	6	NULL	NULL	0	NULL	GATA-4	NULL		bind	NULL				BNP	NULL			promoter	NULL	left ventricle	0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24852_s_292	15051723	A major finding of the present study was that mechanical stretch activated p38 MAPK and that the activation of the kinase was necessary for wall stretch-induced GATA-4 binding to BNP promoter both in the left ventricle and in the atria.	bind
40294	2	10816	6	NULL	NULL	0	NULL	mechanical stretch	NULL		activates	NULL				p38 MAPK	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24852_s_292	15051723	A major finding of the present study was that mechanical stretch activated p38 MAPK and that the activation of the kinase was necessary for wall stretch-induced GATA-4 binding to BNP promoter both in the left ventricle and in the atria.	bind
40295	3	10816	6	NULL	NULL	0	NULL	GATA-4	NULL		bind	NULL				BNP	NULL			promoter	NULL	atria	0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24852_s_292	15051723	A major finding of the present study was that mechanical stretch activated p38 MAPK and that the activation of the kinase was necessary for wall stretch-induced GATA-4 binding to BNP promoter both in the left ventricle and in the atria.	bind
40296	4	10816	6	NULL	NULL	0	NULL	statement 1	NULL		is induced by	NULL				wall stretch	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24852_s_292	15051723	A major finding of the present study was that mechanical stretch activated p38 MAPK and that the activation of the kinase was necessary for wall stretch-induced GATA-4 binding to BNP promoter both in the left ventricle and in the atria.	bind
40297	5	10816	6	NULL	NULL	0	NULL	statement 3	NULL		is induced by	NULL				wall stretch	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24852_s_292	15051723	A major finding of the present study was that mechanical stretch activated p38 MAPK and that the activation of the kinase was necessary for wall stretch-induced GATA-4 binding to BNP promoter both in the left ventricle and in the atria.	bind
40298	6	10816	6	NULL	NULL	0	NULL	statement 2	NULL		is necessary for	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_23_24852_s_292	15051723	A major finding of the present study was that mechanical stretch activated p38 MAPK and that the activation of the kinase was necessary for wall stretch-induced GATA-4 binding to BNP promoter both in the left ventricle and in the atria.	bind
40299	7	10816	6	NULL	NULL	0	NULL	statement 2	NULL		is necessary for	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24852_s_292	15051723	A major finding of the present study was that mechanical stretch activated p38 MAPK and that the activation of the kinase was necessary for wall stretch-induced GATA-4 binding to BNP promoter both in the left ventricle and in the atria.	bind
49781	1	10817	5	13	NULL	NULL	NULL	RanGAP	GP		bind					RanBP2	GP	cytoplasmically oriented			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_4_645_s_38	10330396	A major fraction of RanGAP is bound to the cytoplasmically oriented nucleoporin RanBP2 due to its modification by the ubiquitin-related modifier SUMO-1 (Matunis  et al., 1996  ; Mahajan et al., 1997  ), and the remainder of  RanGAP is soluble in the cytoplasm.	bind
49782	2	10817	5	13	NULL	NULL	NULL	RanBP2	GP		is a type of					nucleoporin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_4_645_s_38	10330396	A major fraction of RanGAP is bound to the cytoplasmically oriented nucleoporin RanBP2 due to its modification by the ubiquitin-related modifier SUMO-1 (Matunis  et al., 1996  ; Mahajan et al., 1997  ), and the remainder of  RanGAP is soluble in the cytoplasm.	bind
49783	3	10817	5	13	NULL	NULL	NULL	RanBP2	GP		is modified by					SUMO-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_4_645_s_38	10330396	A major fraction of RanGAP is bound to the cytoplasmically oriented nucleoporin RanBP2 due to its modification by the ubiquitin-related modifier SUMO-1 (Matunis  et al., 1996  ; Mahajan et al., 1997  ), and the remainder of  RanGAP is soluble in the cytoplasm.	bind
49784	4	10817	5	13	NULL	NULL	NULL	SUMO-1	GP		is a type of					ubiquitin-related modifier	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_4_645_s_38	10330396	A major fraction of RanGAP is bound to the cytoplasmically oriented nucleoporin RanBP2 due to its modification by the ubiquitin-related modifier SUMO-1 (Matunis  et al., 1996  ; Mahajan et al., 1997  ), and the remainder of  RanGAP is soluble in the cytoplasm.	bind
49785	5	10817	5	13	NULL	NULL	NULL	statement 3	Process		leads to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_4_645_s_38	10330396	A major fraction of RanGAP is bound to the cytoplasmically oriented nucleoporin RanBP2 due to its modification by the ubiquitin-related modifier SUMO-1 (Matunis  et al., 1996  ; Mahajan et al., 1997  ), and the remainder of  RanGAP is soluble in the cytoplasm.	bind
49786	6	10817	5	13	NULL	NULL	NULL	RanGAP	GP		is soluble in					cytoplasm	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_4_645_s_38	10330396	A major fraction of RanGAP is bound to the cytoplasmically oriented nucleoporin RanBP2 due to its modification by the ubiquitin-related modifier SUMO-1 (Matunis  et al., 1996  ; Mahajan et al., 1997  ), and the remainder of  RanGAP is soluble in the cytoplasm.	bind
40528	1	10817	6	NULL	NULL	0	NULL	RanGAP	NULL		bind	NULL				RanBP2	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_4_645_s_38	10330396	A major fraction of RanGAP is bound to the cytoplasmically oriented nucleoporin RanBP2 due to its modification by the ubiquitin-related modifier SUMO-1 (Matunis  et al., 1996  ; Mahajan et al., 1997  ), and the remainder of  RanGAP is soluble in the cytoplasm.	bind
40529	2	10817	6	10	NULL	0	NULL	RanBP2			is a type of					cytoplasmically oriented nucleoporin					NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_145_4_645_s_38	10330396	A major fraction of RanGAP is bound to the cytoplasmically oriented nucleoporin RanBP2 due to its modification by the ubiquitin-related modifier SUMO-1 (Matunis  et al., 1996  ; Mahajan et al., 1997  ), and the remainder of  RanGAP is soluble in the cytoplasm.	bind
40530	3	10817	6	NULL	NULL	0	NULL	SUMO-1	NULL		is a type of	NULL				ubiquitin-related modifier	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_4_645_s_38	10330396	A major fraction of RanGAP is bound to the cytoplasmically oriented nucleoporin RanBP2 due to its modification by the ubiquitin-related modifier SUMO-1 (Matunis  et al., 1996  ; Mahajan et al., 1997  ), and the remainder of  RanGAP is soluble in the cytoplasm.	bind
40531	4	10817	6	NULL	NULL	0	NULL	SUMO-1	NULL		modifies	NULL				RanBP2	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_4_645_s_38	10330396	A major fraction of RanGAP is bound to the cytoplasmically oriented nucleoporin RanBP2 due to its modification by the ubiquitin-related modifier SUMO-1 (Matunis  et al., 1996  ; Mahajan et al., 1997  ), and the remainder of  RanGAP is soluble in the cytoplasm.	bind
40532	5	10817	6	NULL	NULL	0	NULL	statement 1	NULL		is because of	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_4_645_s_38	10330396	A major fraction of RanGAP is bound to the cytoplasmically oriented nucleoporin RanBP2 due to its modification by the ubiquitin-related modifier SUMO-1 (Matunis  et al., 1996  ; Mahajan et al., 1997  ), and the remainder of  RanGAP is soluble in the cytoplasm.	bind
40533	6	10817	6	NULL	NULL	0	NULL	RanGAP	NULL		is soluble in	NULL				cytoplasm	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_4_645_s_38	10330396	A major fraction of RanGAP is bound to the cytoplasmically oriented nucleoporin RanBP2 due to its modification by the ubiquitin-related modifier SUMO-1 (Matunis  et al., 1996  ; Mahajan et al., 1997  ), and the remainder of  RanGAP is soluble in the cytoplasm.	bind
49787	1	10818	5	13	NULL	NULL	NULL	trans-acting factor(s)	GP		bind									TCE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_48_37798_s_32	10954723	A major goal of our previous study ( 11) was to identify the  trans-acting factor(s) that bind to the TCE.	bind
40534	1	10818	6	NULL	NULL	0	NULL	trans-acting factor	NULL		bind	NULL					NULL			TCE	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_48_37798_s_32	10954723	A major goal of our previous study ( 11) was to identify the  trans-acting factor(s) that bind to the TCE.	bind
49788	1	10819	5	13	NULL	NULL	NULL	rhodopsin kinase	GP		phosphorylates					rhodopsin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_51_1_161_s_16	9016359	A major mechanism for quenching the visual transduction cascade is initiated by the rapid light-dependent phosphorylation of rhodopsin by the enzyme rhodopsin kinase, followed by the highly selective binding of the protein arrestin to P-Rh* ( 1).	bind
49789	2	10819	5	13	NULL	NULL	NULL	statement 1	Process		is dependent on					light					NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_51_1_161_s_16	9016359	A major mechanism for quenching the visual transduction cascade is initiated by the rapid light-dependent phosphorylation of rhodopsin by the enzyme rhodopsin kinase, followed by the highly selective binding of the protein arrestin to P-Rh* ( 1).	bind
49790	3	10819	5	13	NULL	NULL	NULL	arrestin	GP		bind		highly selective			P-Rh*	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_51_1_161_s_16	9016359	A major mechanism for quenching the visual transduction cascade is initiated by the rapid light-dependent phosphorylation of rhodopsin by the enzyme rhodopsin kinase, followed by the highly selective binding of the protein arrestin to P-Rh* ( 1).	bind
49791	4	10819	5	13	NULL	NULL	NULL	statement 1	Process		is followed by					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_51_1_161_s_16	9016359	A major mechanism for quenching the visual transduction cascade is initiated by the rapid light-dependent phosphorylation of rhodopsin by the enzyme rhodopsin kinase, followed by the highly selective binding of the protein arrestin to P-Rh* ( 1).	bind
49792	5	10819	5	13	NULL	NULL	NULL	statement 4	Process		quenches					visual transduction cascade	Process				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_51_1_161_s_16	9016359	A major mechanism for quenching the visual transduction cascade is initiated by the rapid light-dependent phosphorylation of rhodopsin by the enzyme rhodopsin kinase, followed by the highly selective binding of the protein arrestin to P-Rh* ( 1).	bind
49793	6	10819	5	13	NULL	NULL	NULL	rhodopsin kinase	GP		is a type of					enzyme	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_51_1_161_s_16	9016359	A major mechanism for quenching the visual transduction cascade is initiated by the rapid light-dependent phosphorylation of rhodopsin by the enzyme rhodopsin kinase, followed by the highly selective binding of the protein arrestin to P-Rh* ( 1).	bind
40545	1	10819	6	10	NULL	0	NULL	protein arrestin	NULL		bind	NULL	highly selective			P-Rh*	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_51_1_161_s_16	9016359	A major mechanism for quenching the visual transduction cascade is initiated by the rapid light-dependent phosphorylation of rhodopsin by the enzyme rhodopsin kinase, followed by the highly selective binding of the protein arrestin to P-Rh* ( 1).	bind
40546	2	10819	6	NULL	NULL	0	NULL	rhodopsin kinase	NULL		is a type of	NULL				enzyme	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_51_1_161_s_16	9016359	A major mechanism for quenching the visual transduction cascade is initiated by the rapid light-dependent phosphorylation of rhodopsin by the enzyme rhodopsin kinase, followed by the highly selective binding of the protein arrestin to P-Rh* ( 1).	bind
40547	3	10819	6	NULL	NULL	0	NULL	rhodopsin kinase	NULL		phosphorylates	NULL				rhodopsin	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_51_1_161_s_16	9016359	A major mechanism for quenching the visual transduction cascade is initiated by the rapid light-dependent phosphorylation of rhodopsin by the enzyme rhodopsin kinase, followed by the highly selective binding of the protein arrestin to P-Rh* ( 1).	bind
40548	4	10819	6	NULL	NULL	0	NULL	statement 3	NULL		is dependent on	NULL				light	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_51_1_161_s_16	9016359	A major mechanism for quenching the visual transduction cascade is initiated by the rapid light-dependent phosphorylation of rhodopsin by the enzyme rhodopsin kinase, followed by the highly selective binding of the protein arrestin to P-Rh* ( 1).	bind
40549	5	10819	6	NULL	NULL	0	NULL	statement 4	NULL		quenches	NULL				visual transduction cascade	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_51_1_161_s_16	9016359	A major mechanism for quenching the visual transduction cascade is initiated by the rapid light-dependent phosphorylation of rhodopsin by the enzyme rhodopsin kinase, followed by the highly selective binding of the protein arrestin to P-Rh* ( 1).	bind
50381	6	10819	6	10	NULL	0	NULL	statement 1	NULL		follows	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_51_1_161_s_16	9016359	A major mechanism for quenching the visual transduction cascade is initiated by the rapid light-dependent phosphorylation of rhodopsin by the enzyme rhodopsin kinase, followed by the highly selective binding of the protein arrestin to P-Rh* ( 1).	bind
49794	1	10820	5	13	NULL	NULL	NULL	export cargo protein	GP		bind					CRM1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_1_201_s_146	12529437	A major mechanism of nuclear export involves binding of the export cargo protein to  the exportin CRM1.	bind
49795	2	10820	5	13	NULL	NULL	NULL	CRM1	GP		is a type of					exportin	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_1_201_s_146	12529437	A major mechanism of nuclear export involves binding of the export cargo protein to  the exportin CRM1.	bind
40550	1	10820	6	NULL	NULL	0	NULL	export cargo protein	NULL		bind	NULL				CRM1	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_1_201_s_146	12529437	A major mechanism of nuclear export involves binding of the export cargo protein to  the exportin CRM1.	bind
40551	2	10820	6	NULL	NULL	0	NULL	CRM1	NULL		is a type of	NULL				exportin	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_1_201_s_146	12529437	A major mechanism of nuclear export involves binding of the export cargo protein to  the exportin CRM1.	bind
49796	1	10822	5	13	NULL	NULL	NULL	Mig1	GP		is a type of					zinc finger protein	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_yeast_14_11_9730278_s_2	9730278	A major mediator of glucose repression in yeast is Mig1, a zinc finger  protein that binds to a GC-rich recognition sequence found upstream of  many glucose-repressible genes.	bind
49797	2	10822	5	13	NULL	NULL	NULL	Mig1	GP		mediates					glucose	Chemical	repression of			NULL	yeast	NULL	NULL	NULL	NULL	abs-batch0550-0559_yeast_14_11_9730278_s_2	9730278	A major mediator of glucose repression in yeast is Mig1, a zinc finger  protein that binds to a GC-rich recognition sequence found upstream of  many glucose-repressible genes.	bind
49798	3	10822	5	13	NULL	NULL	NULL	Mig1	GP	yeast	bind					glucose-repressible genes	GP			GC-rich recognition sequence	NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_yeast_14_11_9730278_s_2	9730278	A major mediator of glucose repression in yeast is Mig1, a zinc finger  protein that binds to a GC-rich recognition sequence found upstream of  many glucose-repressible genes.	bind
40552	1	10822	6	NULL	NULL	0	NULL	Mig1	NULL		is a type of	NULL				zinc finger protein	NULL				NULL		0	NULL	NULL	NULL	abs-batch0550-0559_yeast_14_11_9730278_s_2	9730278	A major mediator of glucose repression in yeast is Mig1, a zinc finger  protein that binds to a GC-rich recognition sequence found upstream of  many glucose-repressible genes.	bind
40553	2	10822	6	NULL	NULL	0	NULL	Mig1	NULL		bind	NULL				glucose-repressible gene	NULL			GC-rich recognition sequences	NULL		0	NULL	NULL	NULL	abs-batch0550-0559_yeast_14_11_9730278_s_2	9730278	A major mediator of glucose repression in yeast is Mig1, a zinc finger  protein that binds to a GC-rich recognition sequence found upstream of  many glucose-repressible genes.	bind
40554	3	10822	6	NULL	NULL	0	NULL	Mig1	NULL		mediates	NULL				glucose	NULL	repression of			NULL	yeast	0	NULL	NULL	NULL	abs-batch0550-0559_yeast_14_11_9730278_s_2	9730278	A major mediator of glucose repression in yeast is Mig1, a zinc finger  protein that binds to a GC-rich recognition sequence found upstream of  many glucose-repressible genes.	bind
49799	1	10823	5	13	NULL	NULL	NULL	CITED2	GP		does not bind					TAZ1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_4_3042_s_180	14594809	A major part of the HIF-1alpha binding surface consists of the alphaC helix on the backside of the molecule as viewed in  Fig. 7 A. CITED2 does not contact TAZ1 at all in this region.	bind
40555	1	10823	6	10	NULL	0	NULL	CITED2	NULL		does not bind	NULL				TAZ1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_4_3042_s_180	14594809	A major part of the HIF-1alpha binding surface consists of the alphaC helix on the backside of the molecule as viewed in  Fig. 7 A. CITED2 does not contact TAZ1 at all in this region.	bind
49800	1	10824	5	13	NULL	NULL	NULL	Gsp1p	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0560-0569_embo-j_14_21_7489726_s_4	7489726	A major protein  with the apparent size of 34 kDa co-purifies with the GTP-bound form of  Gsp1p.	bind
40556	1	10824	6	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				Gsp1p	NULL				NULL		0	NULL	NULL	NULL	abs-batch0560-0569_embo-j_14_21_7489726_s_4	7489726	A major protein  with the apparent size of 34 kDa co-purifies with the GTP-bound form of  Gsp1p.	bind
49801	1	10825	5	13	NULL	NULL	NULL	TFIID	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_4_1252_s_2	12582245	A major rate-limiting step in transcription initiation by RNA polymerase II is recognition and binding of the TATA element by the transcription factor TFIID.	bind
49802	2	10825	5	13	NULL	NULL	NULL	TFIID	GP		recognizes									TATA element	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_4_1252_s_2	12582245	A major rate-limiting step in transcription initiation by RNA polymerase II is recognition and binding of the TATA element by the transcription factor TFIID.	bind
49803	3	10825	5	13	NULL	NULL	NULL	TFIID	GP		bind									TATA element	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_4_1252_s_2	12582245	A major rate-limiting step in transcription initiation by RNA polymerase II is recognition and binding of the TATA element by the transcription factor TFIID.	bind
49804	4	10825	5	13	NULL	NULL	NULL	RNA polymerase II	GP		initiates					transcription	Process				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_4_1252_s_2	12582245	A major rate-limiting step in transcription initiation by RNA polymerase II is recognition and binding of the TATA element by the transcription factor TFIID.	bind
49805	5	10825	5	13	NULL	NULL	NULL	statement 4	Process		via					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_4_1252_s_2	12582245	A major rate-limiting step in transcription initiation by RNA polymerase II is recognition and binding of the TATA element by the transcription factor TFIID.	bind
49806	6	10825	5	13	NULL	NULL	NULL	statement 4	Process		via					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_4_1252_s_2	12582245	A major rate-limiting step in transcription initiation by RNA polymerase II is recognition and binding of the TATA element by the transcription factor TFIID.	bind
40557	1	10825	6	NULL	NULL	0	NULL	TFIID	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_31_4_1252_s_2	12582245	A major rate-limiting step in transcription initiation by RNA polymerase II is recognition and binding of the TATA element by the transcription factor TFIID.	bind
40558	2	10825	6	NULL	NULL	0	NULL	TFIID	NULL		bind	NULL					NULL			TATA element	NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_31_4_1252_s_2	12582245	A major rate-limiting step in transcription initiation by RNA polymerase II is recognition and binding of the TATA element by the transcription factor TFIID.	bind
40559	3	10825	6	NULL	NULL	0	NULL	TFIID	NULL		recognizes	NULL					NULL			TATA element	NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_31_4_1252_s_2	12582245	A major rate-limiting step in transcription initiation by RNA polymerase II is recognition and binding of the TATA element by the transcription factor TFIID.	bind
40560	4	10825	6	NULL	NULL	0	NULL	RNA polymerase II	NULL		initiates	NULL				transcription	NULL				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_31_4_1252_s_2	12582245	A major rate-limiting step in transcription initiation by RNA polymerase II is recognition and binding of the TATA element by the transcription factor TFIID.	bind
40561	5	10825	6	NULL	NULL	0	NULL	statement 4	NULL		occurs via	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_31_4_1252_s_2	12582245	A major rate-limiting step in transcription initiation by RNA polymerase II is recognition and binding of the TATA element by the transcription factor TFIID.	bind
40562	6	10825	6	NULL	NULL	0	NULL	statement 4	NULL		occurs via	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_31_4_1252_s_2	12582245	A major rate-limiting step in transcription initiation by RNA polymerase II is recognition and binding of the TATA element by the transcription factor TFIID.	bind
49807	1	10826	5	13	NULL	NULL	NULL	RB	GP		regulates					G1/S transition	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_16_14230_s_78	12584188	A major regulator of G1/S transition is the RB, which binds to the E2F transcription factor, thereby converting E2F from a transcriptional activator to a transcriptional repressor.	bind
49808	2	10826	5	13	NULL	NULL	NULL	RB	GP		bind					E2F	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_16_14230_s_78	12584188	A major regulator of G1/S transition is the RB, which binds to the E2F transcription factor, thereby converting E2F from a transcriptional activator to a transcriptional repressor.	bind
49809	3	10826	5	13	NULL	NULL	NULL	E2F	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_16_14230_s_78	12584188	A major regulator of G1/S transition is the RB, which binds to the E2F transcription factor, thereby converting E2F from a transcriptional activator to a transcriptional repressor.	bind
49810	4	10826	5	13	NULL	NULL	NULL	transcriptional activator	GP		is converted to					transcriptional repressor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_16_14230_s_78	12584188	A major regulator of G1/S transition is the RB, which binds to the E2F transcription factor, thereby converting E2F from a transcriptional activator to a transcriptional repressor.	bind
49811	5	10826	5	13	NULL	NULL	NULL	E2F	GP		is a type of					transcriptional activator	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_16_14230_s_78	12584188	A major regulator of G1/S transition is the RB, which binds to the E2F transcription factor, thereby converting E2F from a transcriptional activator to a transcriptional repressor.	bind
49812	6	10826	5	13	NULL	NULL	NULL	statement 2	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_16_14230_s_78	12584188	A major regulator of G1/S transition is the RB, which binds to the E2F transcription factor, thereby converting E2F from a transcriptional activator to a transcriptional repressor.	bind
40563	1	10826	6	NULL	NULL	0	NULL	RB	NULL		bind	NULL				E2F	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_16_14230_s_78	12584188	A major regulator of G1/S transition is the RB, which binds to the E2F transcription factor, thereby converting E2F from a transcriptional activator to a transcriptional repressor.	bind
40564	2	10826	6	NULL	NULL	0	NULL	E2F	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_16_14230_s_78	12584188	A major regulator of G1/S transition is the RB, which binds to the E2F transcription factor, thereby converting E2F from a transcriptional activator to a transcriptional repressor.	bind
40565	3	10826	6	NULL	NULL	0	NULL	RB	NULL		regulates	NULL				G1/S transition	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_16_14230_s_78	12584188	A major regulator of G1/S transition is the RB, which binds to the E2F transcription factor, thereby converting E2F from a transcriptional activator to a transcriptional repressor.	bind
40566	4	10826	6	NULL	NULL	0	NULL	E2F	NULL		is converted to	NULL				transcriptional repressor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_16_14230_s_78	12584188	A major regulator of G1/S transition is the RB, which binds to the E2F transcription factor, thereby converting E2F from a transcriptional activator to a transcriptional repressor.	bind
40567	5	10826	6	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_16_14230_s_78	12584188	A major regulator of G1/S transition is the RB, which binds to the E2F transcription factor, thereby converting E2F from a transcriptional activator to a transcriptional repressor.	bind
40568	6	10826	6	NULL	NULL	0	NULL	E2F	NULL		is a type of	NULL				transcriptional activator	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_16_14230_s_78	12584188	A major regulator of G1/S transition is the RB, which binds to the E2F transcription factor, thereby converting E2F from a transcriptional activator to a transcriptional repressor.	bind
49815	1	10827	5	13	NULL	NULL	NULL	CmtR	GP		bind		specifically			111-bp P1 fragment	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_45_44560_s_97	12939264	A major retarded complex (and several minor retarded complexes) was formed with increasing concentrations of CmtR with a concomitant decrease in the amount of free probe but no shift of nonspecific competitor DNA ( Fig. 1 D), demonstrating specific binding of CmtR to the 111-bp P1 fragment.	bind
40569	1	10827	6	10	NULL	0	NULL	CmtR	NULL		bind	NULL	specifically			111-bp P1 fragment	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_45_44560_s_97	12939264	A major retarded complex (and several minor retarded complexes) was formed with increasing concentrations of CmtR with a concomitant decrease in the amount of free probe but no shift of nonspecific competitor DNA ( Fig. 1 D), demonstrating specific binding of CmtR to the 111-bp P1 fragment.	bind
49816	1	10828	5	13	NULL	NULL	NULL	TBP	GP		is					TATA-binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1627_2_101_s_3	12818428	A major route to the formation of the preinitiation complex (PIC) for class II transcription  involves the stepwise and ordered assembly of the general transcription factors (GTFs),  initiated by the sequence-specific binding of TATA-binding protein (TBP) (or TFIID)  to the TATA-element in the promoter [  1.	bind
49817	2	10828	5	13	NULL	NULL	NULL	TBP	GP		bind		sequence specifically							TATA-element in promoter	NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1627_2_101_s_3	12818428	A major route to the formation of the preinitiation complex (PIC) for class II transcription  involves the stepwise and ordered assembly of the general transcription factors (GTFs),  initiated by the sequence-specific binding of TATA-binding protein (TBP) (or TFIID)  to the TATA-element in the promoter [  1.	bind
49818	3	10828	5	13	NULL	NULL	NULL	TFIID	GP		bind		sequence specifically							TATA-element in promoter	NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1627_2_101_s_3	12818428	A major route to the formation of the preinitiation complex (PIC) for class II transcription  involves the stepwise and ordered assembly of the general transcription factors (GTFs),  initiated by the sequence-specific binding of TATA-binding protein (TBP) (or TFIID)  to the TATA-element in the promoter [  1.	bind
49819	4	10828	5	13	NULL	NULL	NULL	PIC	GP		is					preinitiation complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1627_2_101_s_3	12818428	A major route to the formation of the preinitiation complex (PIC) for class II transcription  involves the stepwise and ordered assembly of the general transcription factors (GTFs),  initiated by the sequence-specific binding of TATA-binding protein (TBP) (or TFIID)  to the TATA-element in the promoter [  1.	bind
49820	5	10828	5	13	NULL	NULL	NULL	GTFs	GP		is					general transcription factors	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1627_2_101_s_3	12818428	A major route to the formation of the preinitiation complex (PIC) for class II transcription  involves the stepwise and ordered assembly of the general transcription factors (GTFs),  initiated by the sequence-specific binding of TATA-binding protein (TBP) (or TFIID)  to the TATA-element in the promoter [  1.	bind
49821	6	10828	5	13	NULL	NULL	NULL	PIC	GP	formation of	involves					GTFs	GP	stepwise;;ordered assembly of			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1627_2_101_s_3	12818428	A major route to the formation of the preinitiation complex (PIC) for class II transcription  involves the stepwise and ordered assembly of the general transcription factors (GTFs),  initiated by the sequence-specific binding of TATA-binding protein (TBP) (or TFIID)  to the TATA-element in the promoter [  1.	bind
49822	7	10828	5	13	NULL	NULL	NULL	statement 2	Process		initiates					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1627_2_101_s_3	12818428	A major route to the formation of the preinitiation complex (PIC) for class II transcription  involves the stepwise and ordered assembly of the general transcription factors (GTFs),  initiated by the sequence-specific binding of TATA-binding protein (TBP) (or TFIID)  to the TATA-element in the promoter [  1.	bind
49823	8	10828	5	13	NULL	NULL	NULL	statement 3	Process		initiates					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1627_2_101_s_3	12818428	A major route to the formation of the preinitiation complex (PIC) for class II transcription  involves the stepwise and ordered assembly of the general transcription factors (GTFs),  initiated by the sequence-specific binding of TATA-binding protein (TBP) (or TFIID)  to the TATA-element in the promoter [  1.	bind
40570	1	10828	6	NULL	NULL	0	NULL	TBP	NULL		is	NULL				TATA-binding protein	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1627_2_101_s_3	12818428	A major route to the formation of the preinitiation complex (PIC) for class II transcription  involves the stepwise and ordered assembly of the general transcription factors (GTFs),  initiated by the sequence-specific binding of TATA-binding protein (TBP) (or TFIID)  to the TATA-element in the promoter [  1.	bind
40571	2	10828	6	NULL	NULL	0	NULL	TBP	NULL		bind	NULL	sequence specifically				NULL			TATA-element of promoter	NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1627_2_101_s_3	12818428	A major route to the formation of the preinitiation complex (PIC) for class II transcription  involves the stepwise and ordered assembly of the general transcription factors (GTFs),  initiated by the sequence-specific binding of TATA-binding protein (TBP) (or TFIID)  to the TATA-element in the promoter [  1.	bind
40572	3	10828	6	NULL	NULL	0	NULL	TFIID	NULL		bind	NULL	sequence specifically				NULL			TATA-element of promoter	NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1627_2_101_s_3	12818428	A major route to the formation of the preinitiation complex (PIC) for class II transcription  involves the stepwise and ordered assembly of the general transcription factors (GTFs),  initiated by the sequence-specific binding of TATA-binding protein (TBP) (or TFIID)  to the TATA-element in the promoter [  1.	bind
40573	4	10828	6	NULL	NULL	0	NULL	PIC	NULL		is	NULL				preinitiation complex	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1627_2_101_s_3	12818428	A major route to the formation of the preinitiation complex (PIC) for class II transcription  involves the stepwise and ordered assembly of the general transcription factors (GTFs),  initiated by the sequence-specific binding of TATA-binding protein (TBP) (or TFIID)  to the TATA-element in the promoter [  1.	bind
40574	5	10828	6	NULL	NULL	0	NULL	GTF	NULL		is	NULL				general transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1627_2_101_s_3	12818428	A major route to the formation of the preinitiation complex (PIC) for class II transcription  involves the stepwise and ordered assembly of the general transcription factors (GTFs),  initiated by the sequence-specific binding of TATA-binding protein (TBP) (or TFIID)  to the TATA-element in the promoter [  1.	bind
40575	6	10828	6	NULL	NULL	0	NULL	PIC	NULL	formation of	involves	NULL				GTF	NULL	assembly of			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1627_2_101_s_3	12818428	A major route to the formation of the preinitiation complex (PIC) for class II transcription  involves the stepwise and ordered assembly of the general transcription factors (GTFs),  initiated by the sequence-specific binding of TATA-binding protein (TBP) (or TFIID)  to the TATA-element in the promoter [  1.	bind
40576	7	10828	6	NULL	NULL	0	NULL	statement 6	NULL		is initated by	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1627_2_101_s_3	12818428	A major route to the formation of the preinitiation complex (PIC) for class II transcription  involves the stepwise and ordered assembly of the general transcription factors (GTFs),  initiated by the sequence-specific binding of TATA-binding protein (TBP) (or TFIID)  to the TATA-element in the promoter [  1.	bind
40577	8	10828	6	NULL	NULL	0	NULL	statement 6	NULL		is initated by	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1627_2_101_s_3	12818428	A major route to the formation of the preinitiation complex (PIC) for class II transcription  involves the stepwise and ordered assembly of the general transcription factors (GTFs),  initiated by the sequence-specific binding of TATA-binding protein (TBP) (or TFIID)  to the TATA-element in the promoter [  1.	bind
49824	1	10829	5	13	NULL	NULL	NULL	Gab2	GP		is a type of					adapter	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_13_2331_s_244	15933714	A major SHP-2-binding protein is the adapter  Gab2 (  et al), which binds the SH3 domains of Grb2 and Gads (  et al).	bind
49825	2	10829	5	13	NULL	NULL	NULL	Gab2	GP		is a type of					SHP-2-binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_13_2331_s_244	15933714	A major SHP-2-binding protein is the adapter  Gab2 (  et al), which binds the SH3 domains of Grb2 and Gads (  et al).	bind
49826	3	10829	5	13	NULL	NULL	NULL	Gab2	GP		bind					Grb2	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_13_2331_s_244	15933714	A major SHP-2-binding protein is the adapter  Gab2 (  et al), which binds the SH3 domains of Grb2 and Gads (  et al).	bind
49827	4	10829	5	13	NULL	NULL	NULL	Gab2	GP		bind					Gads	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_13_2331_s_244	15933714	A major SHP-2-binding protein is the adapter  Gab2 (  et al), which binds the SH3 domains of Grb2 and Gads (  et al).	bind
40578	1	10829	6	NULL	NULL	0	NULL	Gab2	NULL		bind	NULL				Grb2	NULL		SH3 domain		NULL		0	NULL	NULL	NULL	gw70_embo_24_13_2331_s_244	15933714	A major SHP-2-binding protein is the adapter  Gab2 (  et al), which binds the SH3 domains of Grb2 and Gads (  et al).	bind
40579	2	10829	6	NULL	NULL	0	NULL	Gab2	NULL		bind	NULL				Gads	NULL		SH3 domain		NULL		0	NULL	NULL	NULL	gw70_embo_24_13_2331_s_244	15933714	A major SHP-2-binding protein is the adapter  Gab2 (  et al), which binds the SH3 domains of Grb2 and Gads (  et al).	bind
40580	3	10829	6	NULL	NULL	0	NULL	Gab2	NULL		is a type of	NULL				adapter protein	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_24_13_2331_s_244	15933714	A major SHP-2-binding protein is the adapter  Gab2 (  et al), which binds the SH3 domains of Grb2 and Gads (  et al).	bind
40581	4	10829	6	10	NULL	0	NULL	Gab2	NULL		is a type of	NULL				SHP-2 binding protein	NULL				NULL		NULL	NULL	NULL	NULL	gw70_embo_24_13_2331_s_244	15933714	A major SHP-2-binding protein is the adapter  Gab2 (  et al), which binds the SH3 domains of Grb2 and Gads (  et al).	bind
49828	1	10830	5	13	NULL	NULL	NULL	11 S regulator	GP		bind					20 S proteasome	GP	yeast			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_18_15800_s_215	12600991	A major structural change is induced upon binding of the 11 S regulator to the yeast 20 S proteasome.	bind
49829	2	10830	5	13	NULL	NULL	NULL	statement 1	Process		induce					structural change	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_18_15800_s_215	12600991	A major structural change is induced upon binding of the 11 S regulator to the yeast 20 S proteasome.	bind
40582	1	10830	6	10	NULL	0	NULL	11 S regulator	NULL		bind	NULL				20 S proteasome	NULL	Yeast			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_18_15800_s_215	12600991	A major structural change is induced upon binding of the 11 S regulator to the yeast 20 S proteasome.	bind
40583	2	10830	6	NULL	NULL	0	NULL	statement 1	NULL		induces	NULL				structural change	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_18_15800_s_215	12600991	A major structural change is induced upon binding of the 11 S regulator to the yeast 20 S proteasome.	bind
49830	1	10832	5	13	NULL	NULL	NULL	c-Erb Aalpha1	GP		bind									TREs	NULL	QM7 cells transiently transfected with the T3Ralpha expression vector	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_19_11392_s_123	8626694	A Major T3R-RXR Heterodimer Is Detected in HeLa Cells but  Not in QM7 MyoblastsIn EMSA experiments, we studied the c-Erb  Aalpha1 binding pattern to TREs using QM7 or HeLa cells transiently  transfected with the T3Ralpha  expression vector.	bind
49831	2	10832	5	13	NULL	NULL	NULL	c-Erb Aalpha1	GP		bind									TREs	NULL	HeLa cells transiently transfected with the T3Ralpha expression vector	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_19_11392_s_123	8626694	A Major T3R-RXR Heterodimer Is Detected in HeLa Cells but  Not in QM7 MyoblastsIn EMSA experiments, we studied the c-Erb  Aalpha1 binding pattern to TREs using QM7 or HeLa cells transiently  transfected with the T3Ralpha  expression vector.	bind
40584	1	10832	6	NULL	NULL	0	NULL	c-Erb Aalpha1	NULL		bind	NULL					NULL			TRE	NULL	QM7 transiently transfected with the T3Ralpha expression vector	0	NULL	NULL	NULL	gw60_jbiolchem_271_19_11392_s_123	8626694	A Major T3R-RXR Heterodimer Is Detected in HeLa Cells but  Not in QM7 MyoblastsIn EMSA experiments, we studied the c-Erb  Aalpha1 binding pattern to TREs using QM7 or HeLa cells transiently  transfected with the T3Ralpha  expression vector.	bind
40585	2	10832	6	NULL	NULL	0	NULL	c-Erb Aalpha1	NULL		bind	NULL					NULL			TRE	NULL	HeLa cells transiently transfected with the T3Ralpha expression vector	0	NULL	NULL	NULL	gw60_jbiolchem_271_19_11392_s_123	8626694	A Major T3R-RXR Heterodimer Is Detected in HeLa Cells but  Not in QM7 MyoblastsIn EMSA experiments, we studied the c-Erb  Aalpha1 binding pattern to TREs using QM7 or HeLa cells transiently  transfected with the T3Ralpha  expression vector.	bind
49832	1	10833	5	13	NULL	NULL	NULL	2H-TRE	GP		is					two thyroid hormone response element half-site motifs 	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_biochim-biophys-acta_1761_4_16647292_s_3	16647292	A major transcription start site was identified at -154 bp  relative to the ATG translation initiation codon, within a region containing  two thyroid hormone response element half-site motifs (2H-TRE). Binding  of thyroid hormone receptors alpha and beta1 to this element was demonstrated.	bind
49833	2	10833	5	13	NULL	NULL	NULL	thyroid hormone receptor alpha	GP		bind									2H-TRE	NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_biochim-biophys-acta_1761_4_16647292_s_3	16647292	A major transcription start site was identified at -154 bp  relative to the ATG translation initiation codon, within a region containing  two thyroid hormone response element half-site motifs (2H-TRE). Binding  of thyroid hormone receptors alpha and beta1 to this element was demonstrated.	bind
49834	3	10833	5	13	NULL	NULL	NULL	thyroid hormone receptor beta1	GP		bind									2H-TRE	NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_biochim-biophys-acta_1761_4_16647292_s_3	16647292	A major transcription start site was identified at -154 bp  relative to the ATG translation initiation codon, within a region containing  two thyroid hormone response element half-site motifs (2H-TRE). Binding  of thyroid hormone receptors alpha and beta1 to this element was demonstrated.	bind
40586	1	10833	6	NULL	NULL	0	NULL	2H-TRE	NULL		is	NULL				thyroid hormone response element half-site motif	NULL				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_biochim-biophys-acta_1761_4_16647292_s_3	16647292	A major transcription start site was identified at -154 bp  relative to the ATG translation initiation codon, within a region containing  two thyroid hormone response element half-site motifs (2H-TRE). Binding  of thyroid hormone receptors alpha and beta1 to this element was demonstrated.	bind
40587	2	10833	6	NULL	NULL	0	NULL	thyroid hormone receptor alpha	NULL		bind	NULL					NULL			2H-TRE	NULL		0	NULL	NULL	NULL	abs-batch0700-0719_biochim-biophys-acta_1761_4_16647292_s_3	16647292	A major transcription start site was identified at -154 bp  relative to the ATG translation initiation codon, within a region containing  two thyroid hormone response element half-site motifs (2H-TRE). Binding  of thyroid hormone receptors alpha and beta1 to this element was demonstrated.	bind
40588	3	10833	6	NULL	NULL	0	NULL	thyroid hormone receptor beta1	NULL		bind	NULL					NULL			2H-TRE	NULL		0	NULL	NULL	NULL	abs-batch0700-0719_biochim-biophys-acta_1761_4_16647292_s_3	16647292	A major transcription start site was identified at -154 bp  relative to the ATG translation initiation codon, within a region containing  two thyroid hormone response element half-site motifs (2H-TRE). Binding  of thyroid hormone receptors alpha and beta1 to this element was demonstrated.	bind
49835	1	10834	5	13	NULL	NULL	NULL	SCAP 	GP		bind					insig-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_20_12753_s_248	12242332	A major unresolved question relates to the mechanism by which binding of SCAP to insig-1 or -2 leads to its retention in the ER.	bind
49836	2	10834	5	13	NULL	NULL	NULL	SCAP	GP		bind					insig-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_20_12753_s_248	12242332	A major unresolved question relates to the mechanism by which binding of SCAP to insig-1 or -2 leads to its retention in the ER.	bind
49837	3	10834	5	13	NULL	NULL	NULL	SCAP	GP		is retained in					ER	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_20_12753_s_248	12242332	A major unresolved question relates to the mechanism by which binding of SCAP to insig-1 or -2 leads to its retention in the ER.	bind
49838	4	10834	5	13	NULL	NULL	NULL	statement 1	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_20_12753_s_248	12242332	A major unresolved question relates to the mechanism by which binding of SCAP to insig-1 or -2 leads to its retention in the ER.	bind
49839	5	10834	5	13	NULL	NULL	NULL	statement 2	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_20_12753_s_248	12242332	A major unresolved question relates to the mechanism by which binding of SCAP to insig-1 or -2 leads to its retention in the ER.	bind
40589	1	10834	6	NULL	NULL	0	NULL	SCAP	NULL		bind	NULL				insig-1	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_20_12753_s_248	12242332	A major unresolved question relates to the mechanism by which binding of SCAP to insig-1 or -2 leads to its retention in the ER.	bind
40590	2	10834	6	NULL	NULL	0	NULL	SCAP	NULL		bind	NULL				insig-2	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_20_12753_s_248	12242332	A major unresolved question relates to the mechanism by which binding of SCAP to insig-1 or -2 leads to its retention in the ER.	bind
40591	3	10834	6	NULL	NULL	0	NULL	SCAP	NULL		retains in	NULL				ER	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_20_12753_s_248	12242332	A major unresolved question relates to the mechanism by which binding of SCAP to insig-1 or -2 leads to its retention in the ER.	bind
40592	4	10834	6	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_20_12753_s_248	12242332	A major unresolved question relates to the mechanism by which binding of SCAP to insig-1 or -2 leads to its retention in the ER.	bind
40593	5	10834	6	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_20_12753_s_248	12242332	A major unresolved question relates to the mechanism by which binding of SCAP to insig-1 or -2 leads to its retention in the ER.	bind
49840	1	10837	5	13	NULL	NULL	NULL	maltose binding protein - Kap123p	GP		bind					H2A	GP		NLS		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_153_2_251_s_295	11309407	A maltose binding protein - Kap123p fusion also bound to the H2A and H2B NLSs and not to GST alone (data not shown).	bind
49841	2	10837	5	13	NULL	NULL	NULL	maltose binding protein - Kap123p	GP		bind					H2B	GP		NLS		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_153_2_251_s_295	11309407	A maltose binding protein - Kap123p fusion also bound to the H2A and H2B NLSs and not to GST alone (data not shown).	bind
49842	3	10837	5	13	NULL	NULL	NULL	maltose binding protein - Kap123p	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_153_2_251_s_295	11309407	A maltose binding protein - Kap123p fusion also bound to the H2A and H2B NLSs and not to GST alone (data not shown).	bind
40594	1	10837	6	10	NULL	0	NULL	maltose binding protein - Kap123p 			bind					H2A			NLS		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_153_2_251_s_295	11309407	A maltose binding protein - Kap123p fusion also bound to the H2A and H2B NLSs and not to GST alone (data not shown).	bind
40595	2	10837	6	10	NULL	0	NULL	maltose binding protein - Kap123p 			bind					H2B			NLS		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_153_2_251_s_295	11309407	A maltose binding protein - Kap123p fusion also bound to the H2A and H2B NLSs and not to GST alone (data not shown).	bind
40596	3	10837	6	10	NULL	0	NULL	maltose binding protein - Kap123p 			is a type of					fusion protein					NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_153_2_251_s_295	11309407	A maltose binding protein - Kap123p fusion also bound to the H2A and H2B NLSs and not to GST alone (data not shown).	bind
49843	1	10839	5	13	NULL	NULL	NULL	VP8*	GP		bind					TRAF2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_23_19889_s_134	11262403	A mammalian 2-hybrid analysis was also used to assess VP8* binding to TRAF2 (Fig.  2 B).	bind
40597	1	10839	6	NULL	NULL	0	NULL	VP8*	NULL		bind	NULL				TRAF2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_23_19889_s_134	11262403	A mammalian 2-hybrid analysis was also used to assess VP8* binding to TRAF2 (Fig.  2 B).	bind
49844	1	10840	5	13	NULL	NULL	NULL	Apaf-1	GP		is a type of					CED-4-related caspase adaptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_21_0_71_s_70	12414721	A mammalian CED-4-related caspase adaptor, called Apaf-1, was found ( 70), but unlike CED-4, which binds to CED-9, Apaf-1 did not bind to Bcl-2 (or its homologs)  ( 71).	bind
49845	2	10840	5	13	NULL	NULL	NULL	CED-4	GP		bind					CED-9	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_21_0_71_s_70	12414721	A mammalian CED-4-related caspase adaptor, called Apaf-1, was found ( 70), but unlike CED-4, which binds to CED-9, Apaf-1 did not bind to Bcl-2 (or its homologs)  ( 71).	bind
49846	3	10840	5	13	NULL	NULL	NULL	Apaf-1	GP	mammalian	does not bind					Bcl-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_21_0_71_s_70	12414721	A mammalian CED-4-related caspase adaptor, called Apaf-1, was found ( 70), but unlike CED-4, which binds to CED-9, Apaf-1 did not bind to Bcl-2 (or its homologs)  ( 71).	bind
40598	1	10840	6	NULL	NULL	0	NULL	Apaf-1	NULL		is a type of	NULL				CED-4-related caspase adaptor	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_21_0_71_s_70	12414721	A mammalian CED-4-related caspase adaptor, called Apaf-1, was found ( 70), but unlike CED-4, which binds to CED-9, Apaf-1 did not bind to Bcl-2 (or its homologs)  ( 71).	bind
40599	2	10840	6	NULL	NULL	0	NULL	CED-4	NULL		bind	NULL				CED-9	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_21_0_71_s_70	12414721	A mammalian CED-4-related caspase adaptor, called Apaf-1, was found ( 70), but unlike CED-4, which binds to CED-9, Apaf-1 did not bind to Bcl-2 (or its homologs)  ( 71).	bind
40600	3	10840	6	10	NULL	0	NULL	Apaf-1		mammalian	does not bind					Bcl2					NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_21_0_71_s_70	12414721	A mammalian CED-4-related caspase adaptor, called Apaf-1, was found ( 70), but unlike CED-4, which binds to CED-9, Apaf-1 did not bind to Bcl-2 (or its homologs)  ( 71).	bind
49847	1	10841	5	13	NULL	NULL	NULL	RAFT1	GP		is a type of					FKBP12-rapamycin binding protein	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_genes-dev_10_3_8595879_s_4	8595879	A mammalian FKBP12-rapamycin binding  protein, RAFT1, shares 39% and 43% identity with TOR1 and TOR2 proteins,  respectively but has not been linked to rapamycin action in vivo.	bind
49848	2	10841	5	13	NULL	NULL	NULL	RAFT1	GP	mammalian	is not linked to					rapamycin	Chemical	action of			NULL	in vivo	NULL	NULL	NULL	NULL	abs-batch0517-0529_genes-dev_10_3_8595879_s_4	8595879	A mammalian FKBP12-rapamycin binding  protein, RAFT1, shares 39% and 43% identity with TOR1 and TOR2 proteins,  respectively but has not been linked to rapamycin action in vivo.	bind
50457	3	10841	5	13	NULL	NULL	NULL	RAFT1	GP		is similar to					TOR1 protein	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_genes-dev_10_3_8595879_s_4	8595879	A mammalian FKBP12-rapamycin binding  protein, RAFT1, shares 39% and 43% identity with TOR1 and TOR2 proteins,  respectively but has not been linked to rapamycin action in vivo.	bind
50458	4	10841	5	13	NULL	NULL	NULL	RAFT1	GP		is similar to					TOR2 protein	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_genes-dev_10_3_8595879_s_4	8595879	A mammalian FKBP12-rapamycin binding  protein, RAFT1, shares 39% and 43% identity with TOR1 and TOR2 proteins,  respectively but has not been linked to rapamycin action in vivo.	bind
40601	1	10841	6	NULL	NULL	0	NULL	RAFT1	NULL		is a type of	NULL				FKBP12-rapamycin binding protein	NULL				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_genes-dev_10_3_8595879_s_4	8595879	A mammalian FKBP12-rapamycin binding  protein, RAFT1, shares 39% and 43% identity with TOR1 and TOR2 proteins,  respectively but has not been linked to rapamycin action in vivo.	bind
40602	2	10841	6	10	NULL	0	NULL	RAFT1			is similar to					TOR1 protein					NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_genes-dev_10_3_8595879_s_4	8595879	A mammalian FKBP12-rapamycin binding  protein, RAFT1, shares 39% and 43% identity with TOR1 and TOR2 proteins,  respectively but has not been linked to rapamycin action in vivo.	bind
40603	3	10841	6	10	NULL	0	NULL	RAFT1			is similar to					TOR2 protein					NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_genes-dev_10_3_8595879_s_4	8595879	A mammalian FKBP12-rapamycin binding  protein, RAFT1, shares 39% and 43% identity with TOR1 and TOR2 proteins,  respectively but has not been linked to rapamycin action in vivo.	bind
40604	4	10841	6	10	NULL	0	NULL	RAFT1		mammalian	is not linked to					rapamycin		action of			NULL	in vivo	NULL	NULL	NULL	NULL	abs-batch0517-0529_genes-dev_10_3_8595879_s_4	8595879	A mammalian FKBP12-rapamycin binding  protein, RAFT1, shares 39% and 43% identity with TOR1 and TOR2 proteins,  respectively but has not been linked to rapamycin action in vivo.	bind
49849	1	10842	5	13	NULL	NULL	NULL	guanine nucleotides	NucleicAcid		bind					R-Ras	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_30_18602_s_100	9228027	A mammalian GST-fusion R-Ras expression vector was introduced into COS7 cells and guanine nucleotides bound to R-Ras were examined (Fig.  3,  A and  B).	bind
40605	1	10842	6	NULL	NULL	0	NULL	guanine nucleotides	NULL		bind	NULL				R-Ras	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_30_18602_s_100	9228027	A mammalian GST-fusion R-Ras expression vector was introduced into COS7 cells and guanine nucleotides bound to R-Ras were examined (Fig.  3,  A and  B).	bind
49850	1	10843	5	13	NULL	NULL	NULL	MOB1	GP	mammalian homolog of yeast	is a member of					Striatin Family-Protein Phosphatase 2A Complexes	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_45_31917_s_526	10542219	A Mammalian Homolog of Yeast MOB1 Is Both a Member and a Putative Substrate of Striatin Family-Protein Phosphatase 2A Complexes.	bind
49851	2	10843	5	13	NULL	NULL	NULL	MOB1	GP	mammalian homolog of yeast	is a substrate of		putative			Striatin Family-Protein Phosphatase 2A Complexes	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_45_31917_s_526	10542219	A Mammalian Homolog of Yeast MOB1 Is Both a Member and a Putative Substrate of Striatin Family-Protein Phosphatase 2A Complexes.	bind
40606	1	10843	6	NULL	NULL	0	NULL	MOB1	NULL	mammalian homolog to Yeast	is a member of	NULL				Striatin Family-Protein Phosphatase 2A Complexes	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_45_31917_s_526	10542219	A Mammalian Homolog of Yeast MOB1 Is Both a Member and a Putative Substrate of Striatin Family-Protein Phosphatase 2A Complexes.	bind
40607	2	10843	6	NULL	NULL	0	NULL	MOB1	NULL	mammalian homolog to Yeast	is a substrate for	NULL	putative			Striatin Family-Protein Phosphatase 2A Complexes	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_45_31917_s_526	10542219	A Mammalian Homolog of Yeast MOB1 Is Both a Member and a Putative Substrate of Striatin Family-Protein Phosphatase 2A Complexes.	bind
49852	1	10844	5	13	NULL	NULL	NULL	inscuteable	GP	mammalian partner of	bind					NuMA	GP				NULL		NULL	NULL	NULL	NULL	gw70_nature_437_7056_275_s_265	16094321	A mammalian Partner of inscuteable  binds NuMA and regulates mitotic spindle organization.	bind
49853	2	10844	5	13	NULL	NULL	NULL	statement 1	Process		regulates					mitotic spindle	CellComponent	organization of			NULL		NULL	NULL	NULL	NULL	gw70_nature_437_7056_275_s_265	16094321	A mammalian Partner of inscuteable  binds NuMA and regulates mitotic spindle organization.	bind
40608	1	10844	6	NULL	NULL	0	NULL	inscuteable	NULL	mammalian partner of	bind	NULL				NuMA	NULL				NULL		0	NULL	NULL	NULL	gw70_nature_437_7056_275_s_265	16094321	A mammalian Partner of inscuteable  binds NuMA and regulates mitotic spindle organization.	bind
40609	2	10844	6	10	NULL	0	NULL	statement 1	NULL		regulates	NULL				mitotic spindle 	NULL	organization of			NULL		NULL	NULL	NULL	NULL	gw70_nature_437_7056_275_s_265	16094321	A mammalian Partner of inscuteable  binds NuMA and regulates mitotic spindle organization.	bind
49854	1	10849	5	13	NULL	NULL	NULL	TORs	GP	mammalian homolog of yeast	bind					FKBP12	GP				NULL		NULL	NULL	NULL	NULL	gw60_clinmicrobiolrev_12_4_583_s_2282	10515904	A mammalian protein that binds to FKBP12 in a rapamycin-dependent fashion and is homologous to yeast TORs.	bind
49855	2	10849	5	13	NULL	NULL	NULL	statement 1	Process		is dependent on					rapamycin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_clinmicrobiolrev_12_4_583_s_2282	10515904	A mammalian protein that binds to FKBP12 in a rapamycin-dependent fashion and is homologous to yeast TORs.	bind
40610	1	10849	6	NULL	NULL	0	NULL	TOR	NULL	mammalian homolog to Yeast	bind	NULL				FKBP12	NULL				NULL		0	NULL	NULL	NULL	gw60_clinmicrobiolrev_12_4_583_s_2282	10515904	A mammalian protein that binds to FKBP12 in a rapamycin-dependent fashion and is homologous to yeast TORs.	bind
40611	2	10849	6	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				rapamycin	NULL				NULL		0	NULL	NULL	NULL	gw60_clinmicrobiolrev_12_4_583_s_2282	10515904	A mammalian protein that binds to FKBP12 in a rapamycin-dependent fashion and is homologous to yeast TORs.	bind
49856	1	10852	5	13	NULL	NULL	NULL	VHL peptide	GP	mammalian	bind					Elc1	GP	yeast			NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_16_9033_s_135	10430890	A Mammalian VHL Peptide Binds to Yeast Elc1 and Induces Formation of Two C-Terminal alpha-Helices.	bind
49857	2	10852	5	13	NULL	NULL	NULL	statement 1	Process		induces							formation of	C-Terminal alpha-Helices		NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_16_9033_s_135	10430890	A Mammalian VHL Peptide Binds to Yeast Elc1 and Induces Formation of Two C-Terminal alpha-Helices.	bind
41714	1	10852	6	NULL	NULL	0	NULL	VHL peptide	NULL	mammalian	bind	NULL				Elc1	NULL	Yeast			NULL		0	NULL	NULL	NULL	gw60_pnas_96_16_9033_s_135	10430890	A Mammalian VHL Peptide Binds to Yeast Elc1 and Induces Formation of Two C-Terminal alpha-Helices.	bind
41715	2	10852	6	NULL	NULL	0	NULL	statement 1	NULL		induces	NULL					NULL	formation of	two C-Terminal alpha-Helices		NULL		0	NULL	NULL	NULL	gw60_pnas_96_16_9033_s_135	10430890	A Mammalian VHL Peptide Binds to Yeast Elc1 and Induces Formation of Two C-Terminal alpha-Helices.	bind
49858	1	10853	5	13	NULL	NULL	NULL	N-linked glycopeptide	GP		contains					mannose 6-phosphate	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-immunol_156_5_8596035_s_1	8596035	A mannose 6-phosphate-containing N-linked glycopeptide derived from lysosomal acid lipase is bound to MHC class II in B lymphoblastoid cell lines..	bind
49859	2	10853	5	13	NULL	NULL	NULL	statement 1	GP		bind					MHC class II	GP				NULL	B lymphoblastoid cell lines	NULL	NULL	NULL	NULL	abs-batch0720-0739_j-immunol_156_5_8596035_s_1	8596035	A mannose 6-phosphate-containing N-linked glycopeptide derived from lysosomal acid lipase is bound to MHC class II in B lymphoblastoid cell lines..	bind
49860	3	10853	5	13	NULL	NULL	NULL	statement 1	GP		is derived from					lysosomal acid lipase	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-immunol_156_5_8596035_s_1	8596035	A mannose 6-phosphate-containing N-linked glycopeptide derived from lysosomal acid lipase is bound to MHC class II in B lymphoblastoid cell lines..	bind
41737	1	10853	6	NULL	NULL	0	NULL	N-linked glycopeptide	NULL		contains	NULL				mannose 6-phosphate	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-immunol_156_5_8596035_s_1	8596035	A mannose 6-phosphate-containing N-linked glycopeptide derived from lysosomal acid lipase is bound to MHC class II in B lymphoblastoid cell lines..	bind
41738	2	10853	6	10	NULL	0	NULL	statement 1	NULL		is derived from	NULL				lysosomal acid lipase	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-immunol_156_5_8596035_s_1	8596035	A mannose 6-phosphate-containing N-linked glycopeptide derived from lysosomal acid lipase is bound to MHC class II in B lymphoblastoid cell lines..	bind
41740	3	10853	6	10	NULL	0	NULL	statement 1	NULL		bind	NULL				MHC class II	NULL				NULL	B lymphoblastoid cell lines	NULL	NULL	NULL	NULL	abs-batch0720-0739_j-immunol_156_5_8596035_s_1	8596035	A mannose 6-phosphate-containing N-linked glycopeptide derived from lysosomal acid lipase is bound to MHC class II in B lymphoblastoid cell lines..	bind
49867	1	10857	5	13	NULL	NULL	NULL	3H-DHA	Chemical		bind					beta-adrenoceptors	GP	cortical			NULL	castrated animals	NULL	NULL	NULL	NULL	gw60_jneurosci_21_2_726_s_128	11160451	A marginally significant elevation in the binding of 3H-DHA to cortical beta-adrenoceptors (Fig.  5) was seen for the castrated animals ( F(1,30) = 3.293;  p < 0.08).	bind
41744	1	10857	6	10	NULL	0	NULL	3H-DHA			bind					beta-adrenoceptors		cortical			NULL	castrated animals	NULL	NULL	NULL	NULL	gw60_jneurosci_21_2_726_s_128	11160451	A marginally significant elevation in the binding of 3H-DHA to cortical beta-adrenoceptors (Fig.  5) was seen for the castrated animals ( F(1,30) = 3.293;  p < 0.08).	bind
49868	1	10858	5	13	NULL	NULL	NULL	Cdc27	GP		bind					Nup98	GP				NULL		NULL	NULL	NULL	NULL	gw70_nature_438_7070_1036_s_96	16355229	A marked decrease in Cdc27 and Cdh1 binding to Nup98 occurred in the first 10 min  after nocodazole release, a period when cellular securin started to decline ( Fig. 2g).	bind
49869	2	10858	5	13	NULL	NULL	NULL	Cdh1	GP		bind					Nup98	GP				NULL		NULL	NULL	NULL	NULL	gw70_nature_438_7070_1036_s_96	16355229	A marked decrease in Cdc27 and Cdh1 binding to Nup98 occurred in the first 10 min  after nocodazole release, a period when cellular securin started to decline ( Fig. 2g).	bind
49870	3	10858	5	13	NULL	NULL	NULL	nocodazole	Chemical	release of	decreases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_nature_438_7070_1036_s_96	16355229	A marked decrease in Cdc27 and Cdh1 binding to Nup98 occurred in the first 10 min  after nocodazole release, a period when cellular securin started to decline ( Fig. 2g).	bind
49871	4	10858	5	13	NULL	NULL	NULL	nocodazole	Chemical	release of	decreases					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_nature_438_7070_1036_s_96	16355229	A marked decrease in Cdc27 and Cdh1 binding to Nup98 occurred in the first 10 min  after nocodazole release, a period when cellular securin started to decline ( Fig. 2g).	bind
49872	5	10858	5	13	NULL	NULL	NULL	nocodazole	Chemical	release of	is related to					securin	GP	decline in;;cellular			NULL		NULL	NULL	NULL	NULL	gw70_nature_438_7070_1036_s_96	16355229	A marked decrease in Cdc27 and Cdh1 binding to Nup98 occurred in the first 10 min  after nocodazole release, a period when cellular securin started to decline ( Fig. 2g).	bind
41745	1	10858	6	NULL	NULL	0	NULL	Cdc27	NULL		bind	NULL				Nup98	NULL				NULL		0	NULL	NULL	NULL	gw70_nature_438_7070_1036_s_96	16355229	A marked decrease in Cdc27 and Cdh1 binding to Nup98 occurred in the first 10 min  after nocodazole release, a period when cellular securin started to decline ( Fig. 2g).	bind
41746	2	10858	6	NULL	NULL	0	NULL	Cdh1	NULL		bind	NULL				Nup98	NULL				NULL		0	NULL	NULL	NULL	gw70_nature_438_7070_1036_s_96	16355229	A marked decrease in Cdc27 and Cdh1 binding to Nup98 occurred in the first 10 min  after nocodazole release, a period when cellular securin started to decline ( Fig. 2g).	bind
50459	3	10858	6	10	NULL	0	NULL	nocodazole	NULL	release of	decrease	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_nature_438_7070_1036_s_96	16355229	A marked decrease in Cdc27 and Cdh1 binding to Nup98 occurred in the first 10 min  after nocodazole release, a period when cellular securin started to decline ( Fig. 2g).	bind
50460	4	10858	6	10	NULL	0	NULL	nocodazole	NULL	release of	decrease	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_nature_438_7070_1036_s_96	16355229	A marked decrease in Cdc27 and Cdh1 binding to Nup98 occurred in the first 10 min  after nocodazole release, a period when cellular securin started to decline ( Fig. 2g).	bind
49873	1	10859	5	13	NULL	NULL	NULL	Cdk4	GP		bind					p27	GP				NULL	Tet-p27 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_41_25863_s_92	9325318	A marked increase in p27 levels led only to a small (less than 2-fold) increase in the amount of p27-bound Cdk4 in the Tet-p27 cells (Fig.  1 c), suggesting that most of the cyclin D-Cdk4 present in proliferating Mv1Lu cells is already bound to p27.	bind
49874	2	10859	5	13	NULL	NULL	NULL	p27	GP	increase in	leads to					statement 1	Process	increase in			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_41_25863_s_92	9325318	A marked increase in p27 levels led only to a small (less than 2-fold) increase in the amount of p27-bound Cdk4 in the Tet-p27 cells (Fig.  1 c), suggesting that most of the cyclin D-Cdk4 present in proliferating Mv1Lu cells is already bound to p27.	bind
49876	3	10859	5	13	NULL	NULL	NULL	cyclin D-Cdk4	GP		bind					p27	GP				NULL	proliferating Mv1Lu cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_41_25863_s_92	9325318	A marked increase in p27 levels led only to a small (less than 2-fold) increase in the amount of p27-bound Cdk4 in the Tet-p27 cells (Fig.  1 c), suggesting that most of the cyclin D-Cdk4 present in proliferating Mv1Lu cells is already bound to p27.	bind
41747	1	10859	6	NULL	NULL	0	NULL	p27	NULL		bind	NULL				Cdk4	NULL				NULL	Tet-p27 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_41_25863_s_92	9325318	A marked increase in p27 levels led only to a small (less than 2-fold) increase in the amount of p27-bound Cdk4 in the Tet-p27 cells (Fig.  1 c), suggesting that most of the cyclin D-Cdk4 present in proliferating Mv1Lu cells is already bound to p27.	bind
41748	2	10859	6	NULL	NULL	0	NULL	cyclin D-Cdk4	NULL		bind	NULL				p27	NULL				NULL	proliferating Mv1Lu cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_41_25863_s_92	9325318	A marked increase in p27 levels led only to a small (less than 2-fold) increase in the amount of p27-bound Cdk4 in the Tet-p27 cells (Fig.  1 c), suggesting that most of the cyclin D-Cdk4 present in proliferating Mv1Lu cells is already bound to p27.	bind
42049	3	10859	6	NULL	NULL	0	NULL	p27	NULL	increase in	leads to	NULL				statement 1	NULL	small increase in			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_41_25863_s_92	9325318	A marked increase in p27 levels led only to a small (less than 2-fold) increase in the amount of p27-bound Cdk4 in the Tet-p27 cells (Fig.  1 c), suggesting that most of the cyclin D-Cdk4 present in proliferating Mv1Lu cells is already bound to p27.	bind
49877	1	10861	5	13	NULL	NULL	NULL	E-selectin/IgM	GP		bind					sulfated compounds	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_42_32642_s_204	10938267	A markedly different pattern of E-selectin/IgM binding to the sulfated compounds was observed compared with L-selectingM (Fig.  8 B).	bind
49878	2	10861	5	13	NULL	NULL	NULL	L-selectingM	GP		bind					sulfated compounds	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_42_32642_s_204	10938267	A markedly different pattern of E-selectin/IgM binding to the sulfated compounds was observed compared with L-selectingM (Fig.  8 B).	bind
41749	1	10861	6	NULL	NULL	0	NULL	E-selectin/IgM	NULL		bind	NULL				sulfated compounds	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_42_32642_s_204	10938267	A markedly different pattern of E-selectin/IgM binding to the sulfated compounds was observed compared with L-selectingM (Fig.  8 B).	bind
50461	2	10861	6	10	NULL	0	NULL	 L-selectingM	NULL		bind	NULL				sulfated compounds	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_42_32642_s_204	10938267	A markedly different pattern of E-selectin/IgM binding to the sulfated compounds was observed compared with L-selectingM (Fig.  8 B).	bind
49880	1	10862	5	13	NULL	NULL	NULL	cisplatin	Chemical		bind					transferrin	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_chembiochem_6_10_16196027_s_1	16196027	A mass spectrometric and molecular modelling study of cisplatin binding to transferrin..	bind
41750	1	10862	6	NULL	NULL	0	NULL	cisplatin	NULL		bind	NULL				transferrin	NULL				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_chembiochem_6_10_16196027_s_1	16196027	A mass spectrometric and molecular modelling study of cisplatin binding to transferrin..	bind
49881	1	10863	5	13	NULL	NULL	NULL	Ras	GP		bind					GTP	Chemical				NULL	sensory neurons	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_37_21751_s_98	7665594	A maximally effective  concentration of NGF (1 nM  or 26 ng/ml) was able to stimulate  GTP binding to Ras in both sensory and sympathetic neurons at all  stages examined.	bind
49882	2	10863	5	13	NULL	NULL	NULL	NGF	GP		stimulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_37_21751_s_98	7665594	A maximally effective  concentration of NGF (1 nM  or 26 ng/ml) was able to stimulate  GTP binding to Ras in both sensory and sympathetic neurons at all  stages examined.	bind
50462	3	10863	5	13	NULL	NULL	NULL	Ras	GP		bind					GTP	Chemical				NULL	sympathetic neurons	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_37_21751_s_98	7665594	A maximally effective  concentration of NGF (1 nM  or 26 ng/ml) was able to stimulate  GTP binding to Ras in both sensory and sympathetic neurons at all  stages examined.	bind
50463	4	10863	5	13	NULL	NULL	NULL	NGF	GP		stimulates					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_37_21751_s_98	7665594	A maximally effective  concentration of NGF (1 nM  or 26 ng/ml) was able to stimulate  GTP binding to Ras in both sensory and sympathetic neurons at all  stages examined.	bind
41753	1	10863	6	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				Ras	NULL				NULL	sensory neurons	0	NULL	NULL	NULL	gw60_jbiolchem_270_37_21751_s_98	7665594	A maximally effective  concentration of NGF (1 nM  or 26 ng/ml) was able to stimulate  GTP binding to Ras in both sensory and sympathetic neurons at all  stages examined.	bind
41755	2	10863	6	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				Ras	NULL				NULL	sympathetic neurons	0	NULL	NULL	NULL	gw60_jbiolchem_270_37_21751_s_98	7665594	A maximally effective  concentration of NGF (1 nM  or 26 ng/ml) was able to stimulate  GTP binding to Ras in both sensory and sympathetic neurons at all  stages examined.	bind
41757	3	10863	6	NULL	NULL	0	NULL	NGF	NULL		stimulates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_37_21751_s_98	7665594	A maximally effective  concentration of NGF (1 nM  or 26 ng/ml) was able to stimulate  GTP binding to Ras in both sensory and sympathetic neurons at all  stages examined.	bind
41758	4	10863	6	NULL	NULL	0	NULL	NGF	NULL		stimulates	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_37_21751_s_98	7665594	A maximally effective  concentration of NGF (1 nM  or 26 ng/ml) was able to stimulate  GTP binding to Ras in both sensory and sympathetic neurons at all  stages examined.	bind
49883	1	10864	5	13	NULL	NULL	NULL	eIF4G	GP		bind					eIF3	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_8_1659_s_203	16541103	A maximally effective concentration of insulin had little effect on the amount of  eIF4G bound to eIF3 after 1 min of incubation ( Figure 7A); however, the amount of eIF4G bound was increased more than two-fold after 3 min  ( Figure 7B).	bind
49884	2	10864	5	13	NULL	NULL	NULL	insulin	GP		increases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_8_1659_s_203	16541103	A maximally effective concentration of insulin had little effect on the amount of  eIF4G bound to eIF3 after 1 min of incubation ( Figure 7A); however, the amount of eIF4G bound was increased more than two-fold after 3 min  ( Figure 7B).	bind
41763	1	10864	6	NULL	NULL	0	NULL	eIF4G	NULL		bind	NULL				eIF3	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_25_8_1659_s_203	16541103	A maximally effective concentration of insulin had little effect on the amount of  eIF4G bound to eIF3 after 1 min of incubation ( Figure 7A); however, the amount of eIF4G bound was increased more than two-fold after 3 min  ( Figure 7B).	bind
41765	2	10864	6	10	NULL	0	NULL	insulin	NULL		increases	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_8_1659_s_203	16541103	A maximally effective concentration of insulin had little effect on the amount of  eIF4G bound to eIF3 after 1 min of incubation ( Figure 7A); however, the amount of eIF4G bound was increased more than two-fold after 3 min  ( Figure 7B).	bind
49885	1	10865	5	13	NULL	NULL	NULL	E1	GP		bind					E2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_8_6921_s_356	14638692	A maximum  S* value of 81  plus-or-minus  1 S is reached which is 18.4 S below that with saturated binding of  E1 to  E2	bind
41783	1	10865	6	NULL	NULL	0	NULL	E1	NULL		bind	NULL				E2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_6921_s_356	14638692	A maximum  S* value of 81  plus-or-minus  1 S is reached which is 18.4 S below that with saturated binding of  E1 to  E2	bind
49886	1	10867	5	13	NULL	NULL	NULL	water molecule	Chemical		bind					tyrosine-9	AminoAcid				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochem-biophys-res-commun_280_3_11162605_s_8	11162605	A mechanism  involving a tyrosine-9-bound water molecule acting as a proton shuttle  is proposed for the Michael additions catalyzed by GST A4-4.	bind
49887	2	10867	5	13	NULL	NULL	NULL	statement 1	Process		acts as					proton shuttle	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochem-biophys-res-commun_280_3_11162605_s_8	11162605	A mechanism  involving a tyrosine-9-bound water molecule acting as a proton shuttle  is proposed for the Michael additions catalyzed by GST A4-4.	bind
41789	1	10867	6	10	NULL	0	NULL	tyrosine-9			bind					water molecule					NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochem-biophys-res-commun_280_3_11162605_s_8	11162605	A mechanism  involving a tyrosine-9-bound water molecule acting as a proton shuttle  is proposed for the Michael additions catalyzed by GST A4-4.	bind
50464	2	10867	6	10	NULL	0	NULL	statement 1	NULL		acts as a	NULL				proton shuttle	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_biochem-biophys-res-commun_280_3_11162605_s_8	11162605	A mechanism  involving a tyrosine-9-bound water molecule acting as a proton shuttle  is proposed for the Michael additions catalyzed by GST A4-4.	bind
49888	1	10868	5	13	NULL	NULL	NULL	NC2	GP	heterodimeric 	bind			histone fold domains		TBP-promoter complexes	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_34_0_77_s_1658	11092823	A mechanism for  repression of class II gene transcription through specific binding of NC2 to TBP-promoter  complexes via heterodimeric histone fold domains.	bind
49889	2	10868	5	13	NULL	NULL	NULL	statement 1	Process		repress					class II gene	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_34_0_77_s_1658	11092823	A mechanism for  repression of class II gene transcription through specific binding of NC2 to TBP-promoter  complexes via heterodimeric histone fold domains.	bind
41796	1	10868	6	10	NULL	0	NULL	NC2		heterodimeric	bind			histone fold domains		TBP-promoter complex					NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_34_0_77_s_1658	11092823	A mechanism for  repression of class II gene transcription through specific binding of NC2 to TBP-promoter  complexes via heterodimeric histone fold domains.	bind
41798	2	10868	6	NULL	NULL	0	NULL	statement 1	NULL		represses	NULL				class II gene	NULL	transcription of 			NULL		0	NULL	NULL	NULL	gw70_annurevgenet_34_0_77_s_1658	11092823	A mechanism for  repression of class II gene transcription through specific binding of NC2 to TBP-promoter  complexes via heterodimeric histone fold domains.	bind
49890	1	10869	5	13	NULL	NULL	NULL	QacR dimers	GP		bind		cooperatively			IR1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_24_7102_s_219	11717268	A mechanism for cooperative binding of QacR dimers to IR1 that involved indirect interactions through the DNA would be consistent with all the results presented in this work.	bind
41799	1	10869	6	NULL	NULL	0	NULL	QacR dimers	NULL		bind	NULL	cooperatively			IR1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_24_7102_s_219	11717268	A mechanism for cooperative binding of QacR dimers to IR1 that involved indirect interactions through the DNA would be consistent with all the results presented in this work.	bind
49891	1	10876	5	13	NULL	NULL	NULL	BAR	GP		induce					SHP	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_9_7027_s_28	12496277	A mechanism has been proposed whereby BAR induces the negative transcriptional regulator  SHP (small heterodimer partner), which in turn represses transcription factors that bind to the  CYP7A1 BAREs ( ,  ).	bind
49892	2	10876	5	13	NULL	NULL	NULL	SHP	GP		is					small heterodimer partner	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_9_7027_s_28	12496277	A mechanism has been proposed whereby BAR induces the negative transcriptional regulator  SHP (small heterodimer partner), which in turn represses transcription factors that bind to the  CYP7A1 BAREs ( ,  ).	bind
49893	3	10876	5	13	NULL	NULL	NULL	SHP	GP		is a type of					negative transcriptional regulator	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_9_7027_s_28	12496277	A mechanism has been proposed whereby BAR induces the negative transcriptional regulator  SHP (small heterodimer partner), which in turn represses transcription factors that bind to the  CYP7A1 BAREs ( ,  ).	bind
49894	4	10876	5	13	NULL	NULL	NULL	transcription factors	GP		bind					CYP7A1	GP			BAREs	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_9_7027_s_28	12496277	A mechanism has been proposed whereby BAR induces the negative transcriptional regulator  SHP (small heterodimer partner), which in turn represses transcription factors that bind to the  CYP7A1 BAREs ( ,  ).	bind
49895	5	10876	5	13	NULL	NULL	NULL	SHP	GP		repress					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_9_7027_s_28	12496277	A mechanism has been proposed whereby BAR induces the negative transcriptional regulator  SHP (small heterodimer partner), which in turn represses transcription factors that bind to the  CYP7A1 BAREs ( ,  ).	bind
49896	6	10876	5	13	NULL	NULL	NULL	statement 1	Process		leads to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_9_7027_s_28	12496277	A mechanism has been proposed whereby BAR induces the negative transcriptional regulator  SHP (small heterodimer partner), which in turn represses transcription factors that bind to the  CYP7A1 BAREs ( ,  ).	bind
41834	1	10876	6	10	NULL	0	NULL	transcription factor	NULL		bind	NULL				CYP7A1	NULL			BARE	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_9_7027_s_28	12496277	A mechanism has been proposed whereby BAR induces the negative transcriptional regulator  SHP (small heterodimer partner), which in turn represses transcription factors that bind to the  CYP7A1 BAREs ( ,  ).	bind
41835	2	10876	6	NULL	NULL	0	NULL	SHP	NULL		represses	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_9_7027_s_28	12496277	A mechanism has been proposed whereby BAR induces the negative transcriptional regulator  SHP (small heterodimer partner), which in turn represses transcription factors that bind to the  CYP7A1 BAREs ( ,  ).	bind
41836	3	10876	6	10	NULL	0	NULL	SHP	NULL		is a type of	NULL				negative transcriptional regulator	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_9_7027_s_28	12496277	A mechanism has been proposed whereby BAR induces the negative transcriptional regulator  SHP (small heterodimer partner), which in turn represses transcription factors that bind to the  CYP7A1 BAREs ( ,  ).	bind
41837	4	10876	6	NULL	NULL	0	NULL	BAR	NULL		induces	NULL				SHP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_9_7027_s_28	12496277	A mechanism has been proposed whereby BAR induces the negative transcriptional regulator  SHP (small heterodimer partner), which in turn represses transcription factors that bind to the  CYP7A1 BAREs ( ,  ).	bind
41838	5	10876	6	NULL	NULL	0	NULL	SHP	NULL		is	NULL				small heterodimer partner	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_9_7027_s_28	12496277	A mechanism has been proposed whereby BAR induces the negative transcriptional regulator  SHP (small heterodimer partner), which in turn represses transcription factors that bind to the  CYP7A1 BAREs ( ,  ).	bind
50465	6	10876	6	10	NULL	0	NULL	statement 4	NULL		leads to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_9_7027_s_28	12496277	A mechanism has been proposed whereby BAR induces the negative transcriptional regulator  SHP (small heterodimer partner), which in turn represses transcription factors that bind to the  CYP7A1 BAREs ( ,  ).	bind
49897	1	10878	5	13	NULL	NULL	NULL	KCNK3	GP		is a type of					channel	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_111_4_577_s_22	12437930	A mechanism is suggested by demonstration that (despite separation of retention and release motifs in the KCNK3 primary sequence) the channels bind beta-COP or 14-3-3beta in mutually exclusive fashion.	bind
49898	2	10878	5	13	NULL	NULL	NULL	KCNK3	GP		bind					beta-COP	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_111_4_577_s_22	12437930	A mechanism is suggested by demonstration that (despite separation of retention and release motifs in the KCNK3 primary sequence) the channels bind beta-COP or 14-3-3beta in mutually exclusive fashion.	bind
49899	3	10878	5	13	NULL	NULL	NULL	KCNK3	GP		bind					14-3-3beta	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_111_4_577_s_22	12437930	A mechanism is suggested by demonstration that (despite separation of retention and release motifs in the KCNK3 primary sequence) the channels bind beta-COP or 14-3-3beta in mutually exclusive fashion.	bind
49900	4	10878	5	13	NULL	NULL	NULL	statement 2	Process		mutually exclusive to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_111_4_577_s_22	12437930	A mechanism is suggested by demonstration that (despite separation of retention and release motifs in the KCNK3 primary sequence) the channels bind beta-COP or 14-3-3beta in mutually exclusive fashion.	bind
41856	1	10878	6	NULL	NULL	0	NULL	KCNK3	NULL		is a type of	NULL				channel	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_111_4_577_s_22	12437930	A mechanism is suggested by demonstration that (despite separation of retention and release motifs in the KCNK3 primary sequence) the channels bind beta-COP or 14-3-3beta in mutually exclusive fashion.	bind
41858	2	10878	6	NULL	NULL	0	NULL	KCNK3	NULL		bind	NULL				beta-COP	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_111_4_577_s_22	12437930	A mechanism is suggested by demonstration that (despite separation of retention and release motifs in the KCNK3 primary sequence) the channels bind beta-COP or 14-3-3beta in mutually exclusive fashion.	bind
41859	3	10878	6	NULL	NULL	0	NULL	KCNK3	NULL		bind	NULL				14-3-3beta	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_111_4_577_s_22	12437930	A mechanism is suggested by demonstration that (despite separation of retention and release motifs in the KCNK3 primary sequence) the channels bind beta-COP or 14-3-3beta in mutually exclusive fashion.	bind
41860	4	10878	6	NULL	NULL	0	NULL	statement 2	NULL		is independent of	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_111_4_577_s_22	12437930	A mechanism is suggested by demonstration that (despite separation of retention and release motifs in the KCNK3 primary sequence) the channels bind beta-COP or 14-3-3beta in mutually exclusive fashion.	bind
49901	1	10879	5	13	NULL	NULL	NULL	Spi-1	GP		bind			wHTH domain		IL1B	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_294_4_854_s_134	12061786	A mechanism of PTT was suggested in which the Spi-1 wHTH domain binds to the  IL1B promoter and physically interacts with IE2, which provides both TBP recruitment and acidic transactivation domains.	bind
49902	2	10879	5	13	NULL	NULL	NULL	Spi-1	GP		interacts with		physically	wHTH domain		IE2	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_294_4_854_s_134	12061786	A mechanism of PTT was suggested in which the Spi-1 wHTH domain binds to the  IL1B promoter and physically interacts with IE2, which provides both TBP recruitment and acidic transactivation domains.	bind
49903	3	10879	5	13	NULL	NULL	NULL	statement 2	Process		leads to					TBP	GP	recruitment of			NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_294_4_854_s_134	12061786	A mechanism of PTT was suggested in which the Spi-1 wHTH domain binds to the  IL1B promoter and physically interacts with IE2, which provides both TBP recruitment and acidic transactivation domains.	bind
50466	4	10879	5	13	NULL	NULL	NULL	statement 2	Process		leads to							acidic	transactivation domain		NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_294_4_854_s_134	12061786	A mechanism of PTT was suggested in which the Spi-1 wHTH domain binds to the  IL1B promoter and physically interacts with IE2, which provides both TBP recruitment and acidic transactivation domains.	bind
41908	1	10879	6	NULL	NULL	0	NULL	Spi-1	NULL		bind	NULL		wHTH domain		IL1B	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_294_4_854_s_134	12061786	A mechanism of PTT was suggested in which the Spi-1 wHTH domain binds to the  IL1B promoter and physically interacts with IE2, which provides both TBP recruitment and acidic transactivation domains.	bind
41909	2	10879	6	10	NULL	0	NULL	Spi-1	NULL		interacts with	NULL	physically	wHTH domain		IE2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_294_4_854_s_134	12061786	A mechanism of PTT was suggested in which the Spi-1 wHTH domain binds to the  IL1B promoter and physically interacts with IE2, which provides both TBP recruitment and acidic transactivation domains.	bind
41910	3	10879	6	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				TBP	NULL	recruitment of			NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_294_4_854_s_134	12061786	A mechanism of PTT was suggested in which the Spi-1 wHTH domain binds to the  IL1B promoter and physically interacts with IE2, which provides both TBP recruitment and acidic transactivation domains.	bind
41911	4	10879	6	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL					NULL	acidic	transactivation domain		NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_294_4_854_s_134	12061786	A mechanism of PTT was suggested in which the Spi-1 wHTH domain binds to the  IL1B promoter and physically interacts with IE2, which provides both TBP recruitment and acidic transactivation domains.	bind
49904	1	10880	5	13	NULL	NULL	NULL	OxyR 	GP		bind					mom	GP			GATC sites	NULL		NULL	NULL	NULL	NULL	gw60_genetics_152_1_31_s_435	10408954	A mechanism of this kind would be analogous to that described for  mom, with the difference that OxyR binds to GATC sites located upstream of the  mom promoter ( B OLKER and KAHMANN 1989   ).	bind
49905	2	10880	5	13	NULL	NULL	NULL				is located				GATC sites	mom	GP	upstream of		promoter	NULL		NULL	NULL	NULL	NULL	gw60_genetics_152_1_31_s_435	10408954	A mechanism of this kind would be analogous to that described for  mom, with the difference that OxyR binds to GATC sites located upstream of the  mom promoter ( B OLKER and KAHMANN 1989   ).	bind
41912	1	10880	6	10	NULL	0	NULL	OxyR	NULL		bind	NULL				mom	NULL			GATC sites 	NULL		NULL	NULL	NULL	NULL	gw60_genetics_152_1_31_s_435	10408954	A mechanism of this kind would be analogous to that described for  mom, with the difference that OxyR binds to GATC sites located upstream of the  mom promoter ( B OLKER and KAHMANN 1989   ).	bind
50467	2	10880	6	10	NULL	0	NULL		NULL		is located 	NULL			GATC sites	mom	NULL	upstream of		promoter	NULL		0	NULL	NULL	NULL	gw60_genetics_152_1_31_s_435	10408954	A mechanism of this kind would be analogous to that described for  mom, with the difference that OxyR binds to GATC sites located upstream of the  mom promoter ( B OLKER and KAHMANN 1989   ).	bind
49906	1	10881	5	13	NULL	NULL	NULL	Hsp70	GP		bind					HSF1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_17_12081_s_175	10207033	A mechanism that has been proposed for autoregulation or self-limiting expression of  Hsp70 is based on the observation that Hsp70 binds to HSF1 ( 20-22).	bind
41913	1	10881	6	NULL	NULL	0	NULL	Hsp70	NULL		bind	NULL				HSF1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_17_12081_s_175	10207033	A mechanism that has been proposed for autoregulation or self-limiting expression of  Hsp70 is based on the observation that Hsp70 binds to HSF1 ( 20-22).	bind
49907	1	10882	5	13	NULL	NULL	NULL	chaperone	GP		is involved in					Cxs	GP	membrane integration of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_14_7856_s_250	9525879	A mechanism that would explain this phenomenon is that a specific factor, such as a chaperone that normally is involved in the membrane integration of Cxs and, for example, binds to the Cx polypeptide sequence to aid in their correct positioning within the ER translocon (represented schematically in Fig.  8 C), is absent or not functional in the cell-free expression system.	bind
49908	2	10882	5	13	NULL	NULL	NULL	chaperone	GP		bind					Cx polypeptide sequence	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_14_7856_s_250	9525879	A mechanism that would explain this phenomenon is that a specific factor, such as a chaperone that normally is involved in the membrane integration of Cxs and, for example, binds to the Cx polypeptide sequence to aid in their correct positioning within the ER translocon (represented schematically in Fig.  8 C), is absent or not functional in the cell-free expression system.	bind
49909	3	10882	5	13	NULL	NULL	NULL	chaperone	GP		is positioned within					ER translocon	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_14_7856_s_250	9525879	A mechanism that would explain this phenomenon is that a specific factor, such as a chaperone that normally is involved in the membrane integration of Cxs and, for example, binds to the Cx polypeptide sequence to aid in their correct positioning within the ER translocon (represented schematically in Fig.  8 C), is absent or not functional in the cell-free expression system.	bind
49910	4	10882	5	13	NULL	NULL	NULL	statement 2	Process		aid in					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_14_7856_s_250	9525879	A mechanism that would explain this phenomenon is that a specific factor, such as a chaperone that normally is involved in the membrane integration of Cxs and, for example, binds to the Cx polypeptide sequence to aid in their correct positioning within the ER translocon (represented schematically in Fig.  8 C), is absent or not functional in the cell-free expression system.	bind
42050	1	10882	6	NULL	NULL	0	NULL	chaperone	NULL		is involved in	NULL				Cxs	NULL	membrane integration of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_7856_s_250	9525879	A mechanism that would explain this phenomenon is that a specific factor, such as a chaperone that normally is involved in the membrane integration of Cxs and, for example, binds to the Cx polypeptide sequence to aid in their correct positioning within the ER translocon (represented schematically in Fig.  8 C), is absent or not functional in the cell-free expression system.	bind
42051	2	10882	6	NULL	NULL	0	NULL	chaperone	NULL		is positioned within	NULL				ER translocon	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_7856_s_250	9525879	A mechanism that would explain this phenomenon is that a specific factor, such as a chaperone that normally is involved in the membrane integration of Cxs and, for example, binds to the Cx polypeptide sequence to aid in their correct positioning within the ER translocon (represented schematically in Fig.  8 C), is absent or not functional in the cell-free expression system.	bind
42052	3	10882	6	NULL	NULL	0	NULL	chaperone	NULL		bind	NULL				Cx polypeptide	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_7856_s_250	9525879	A mechanism that would explain this phenomenon is that a specific factor, such as a chaperone that normally is involved in the membrane integration of Cxs and, for example, binds to the Cx polypeptide sequence to aid in their correct positioning within the ER translocon (represented schematically in Fig.  8 C), is absent or not functional in the cell-free expression system.	bind
42053	4	10882	6	NULL	NULL	0	NULL	statement 3	NULL		aids in	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_7856_s_250	9525879	A mechanism that would explain this phenomenon is that a specific factor, such as a chaperone that normally is involved in the membrane integration of Cxs and, for example, binds to the Cx polypeptide sequence to aid in their correct positioning within the ER translocon (represented schematically in Fig.  8 C), is absent or not functional in the cell-free expression system.	bind
49911	1	10883	5	13	NULL	NULL	NULL	synaptobrevin	GP		bind			S1 domain		exosites	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_6_3459_s_133	9013591	A mechanism which could account for the present results is the promotion of an active conformation of TeNT induced by the binding of the S1 and S2 domains of synaptobrevin to exosites present on the toxin surface, as in the case of allosteric enzymes ( 36-38).	bind
49912	2	10883	5	13	NULL	NULL	NULL	exosites	Chemical		is present on					toxin	Chemical	surface of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_6_3459_s_133	9013591	A mechanism which could account for the present results is the promotion of an active conformation of TeNT induced by the binding of the S1 and S2 domains of synaptobrevin to exosites present on the toxin surface, as in the case of allosteric enzymes ( 36-38).	bind
49913	3	10883	5	13	NULL	NULL	NULL	synaptobrevin	GP		bind			S2 domain		exosites 	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_6_3459_s_133	9013591	A mechanism which could account for the present results is the promotion of an active conformation of TeNT induced by the binding of the S1 and S2 domains of synaptobrevin to exosites present on the toxin surface, as in the case of allosteric enzymes ( 36-38).	bind
49914	4	10883	5	13	NULL	NULL	NULL	statement 1	Process		induce					TeNT	GP	active conformation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_6_3459_s_133	9013591	A mechanism which could account for the present results is the promotion of an active conformation of TeNT induced by the binding of the S1 and S2 domains of synaptobrevin to exosites present on the toxin surface, as in the case of allosteric enzymes ( 36-38).	bind
49915	5	10883	5	13	NULL	NULL	NULL	statement 3	Process		induce					TeNT	GP	active conformation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_6_3459_s_133	9013591	A mechanism which could account for the present results is the promotion of an active conformation of TeNT induced by the binding of the S1 and S2 domains of synaptobrevin to exosites present on the toxin surface, as in the case of allosteric enzymes ( 36-38).	bind
41914	1	10883	6	10	NULL	0	NULL	exosite	NULL		is present on	NULL				toxin surface	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_6_3459_s_133	9013591	A mechanism which could account for the present results is the promotion of an active conformation of TeNT induced by the binding of the S1 and S2 domains of synaptobrevin to exosites present on the toxin surface, as in the case of allosteric enzymes ( 36-38).	bind
41915	2	10883	6	10	NULL	0	NULL	synaptobrevin	NULL		bind	NULL		S1 domain		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_6_3459_s_133	9013591	A mechanism which could account for the present results is the promotion of an active conformation of TeNT induced by the binding of the S1 and S2 domains of synaptobrevin to exosites present on the toxin surface, as in the case of allosteric enzymes ( 36-38).	bind
41916	4	10883	6	10	NULL	0	NULL	statement 2	NULL		induces	NULL				TeNT	NULL	active conformation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_6_3459_s_133	9013591	A mechanism which could account for the present results is the promotion of an active conformation of TeNT induced by the binding of the S1 and S2 domains of synaptobrevin to exosites present on the toxin surface, as in the case of allosteric enzymes ( 36-38).	bind
41917	5	10883	6	10	NULL	0	NULL	statement 3	NULL		induces	NULL				TeNT	NULL	active conformation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_6_3459_s_133	9013591	A mechanism which could account for the present results is the promotion of an active conformation of TeNT induced by the binding of the S1 and S2 domains of synaptobrevin to exosites present on the toxin surface, as in the case of allosteric enzymes ( 36-38).	bind
50468	3	10883	6	10	NULL	0	NULL	synaptobrevin	NULL		bind	NULL		S2 domain		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_6_3459_s_133	9013591	A mechanism which could account for the present results is the promotion of an active conformation of TeNT induced by the binding of the S1 and S2 domains of synaptobrevin to exosites present on the toxin surface, as in the case of allosteric enzymes ( 36-38).	bind
49916	1	10884	5	13	NULL	NULL	NULL	PKCs	GP	atypical	bind					p62	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_35344_s_227	11445585	A mechanistic explanation to the roles of atypical PKCs in NF-kappaB activation has been provided by the findings that atypical PKCs bind to the scaffold protein p62 via protein complex formation with receptor interacting protein or TRAF6 in TNF-alpha- or IL-1beta-signaling, respectively ( 39,  81).	bind
49917	2	10884	5	13	NULL	NULL	NULL	p62	GP		is a type of					scaffold protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_35344_s_227	11445585	A mechanistic explanation to the roles of atypical PKCs in NF-kappaB activation has been provided by the findings that atypical PKCs bind to the scaffold protein p62 via protein complex formation with receptor interacting protein or TRAF6 in TNF-alpha- or IL-1beta-signaling, respectively ( 39,  81).	bind
49918	3	10884	5	13	NULL	NULL	NULL	statement 1	Process		via					TRAF6	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_35344_s_227	11445585	A mechanistic explanation to the roles of atypical PKCs in NF-kappaB activation has been provided by the findings that atypical PKCs bind to the scaffold protein p62 via protein complex formation with receptor interacting protein or TRAF6 in TNF-alpha- or IL-1beta-signaling, respectively ( 39,  81).	bind
49919	4	10884	5	13	NULL	NULL	NULL	statement 3	Process		occurs during					IL-1beta	GP	signaling of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_35344_s_227	11445585	A mechanistic explanation to the roles of atypical PKCs in NF-kappaB activation has been provided by the findings that atypical PKCs bind to the scaffold protein p62 via protein complex formation with receptor interacting protein or TRAF6 in TNF-alpha- or IL-1beta-signaling, respectively ( 39,  81).	bind
42054	1	10884	6	NULL	NULL	0	NULL	PKC	NULL	atypical	bind	NULL				p62	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_38_35344_s_227	11445585	A mechanistic explanation to the roles of atypical PKCs in NF-kappaB activation has been provided by the findings that atypical PKCs bind to the scaffold protein p62 via protein complex formation with receptor interacting protein or TRAF6 in TNF-alpha- or IL-1beta-signaling, respectively ( 39,  81).	bind
42055	2	10884	6	NULL	NULL	0	NULL	p62	NULL		is a type of	NULL				scaffold protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_38_35344_s_227	11445585	A mechanistic explanation to the roles of atypical PKCs in NF-kappaB activation has been provided by the findings that atypical PKCs bind to the scaffold protein p62 via protein complex formation with receptor interacting protein or TRAF6 in TNF-alpha- or IL-1beta-signaling, respectively ( 39,  81).	bind
42057	3	10884	6	10	NULL	0	NULL	statement 1	NULL		occurs via	NULL				TRAF6	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_35344_s_227	11445585	A mechanistic explanation to the roles of atypical PKCs in NF-kappaB activation has been provided by the findings that atypical PKCs bind to the scaffold protein p62 via protein complex formation with receptor interacting protein or TRAF6 in TNF-alpha- or IL-1beta-signaling, respectively ( 39,  81).	bind
42058	4	10884	6	10	NULL	0	NULL	statement 3	NULL		occurs during	NULL				IL-1beta	NULL	signaling of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_38_35344_s_227	11445585	A mechanistic explanation to the roles of atypical PKCs in NF-kappaB activation has been provided by the findings that atypical PKCs bind to the scaffold protein p62 via protein complex formation with receptor interacting protein or TRAF6 in TNF-alpha- or IL-1beta-signaling, respectively ( 39,  81).	bind
49922	1	10885	5	13	NULL	NULL	NULL	TFIID complex	GP		bind									promoter	NULL		NULL	NULL	NULL	NULL	gw60_embo_17_17_5103_s_13	9724646	A mechanistic study supported the hypothesis that PC4 facilitates binding of the TFIID complex to promoters (Kaiser  et al., 1995  ).	bind
49923	2	10885	5	13	NULL	NULL	NULL	PC4	GP		facilitates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_17_5103_s_13	9724646	A mechanistic study supported the hypothesis that PC4 facilitates binding of the TFIID complex to promoters (Kaiser  et al., 1995  ).	bind
41918	1	10885	6	NULL	NULL	0	NULL	TFIID complex	NULL		bind	NULL					NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_embo_17_17_5103_s_13	9724646	A mechanistic study supported the hypothesis that PC4 facilitates binding of the TFIID complex to promoters (Kaiser  et al., 1995  ).	bind
41919	2	10885	6	NULL	NULL	0	NULL	PC4	NULL		facilitates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_17_17_5103_s_13	9724646	A mechanistic study supported the hypothesis that PC4 facilitates binding of the TFIID complex to promoters (Kaiser  et al., 1995  ).	bind
49924	1	10886	5	13	NULL	NULL	NULL	CRF	GP		is					corticotropin-releasing factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_brainres_980_2_206_s_337	12867260	A member of the  corticotropin-releasing factor (CRF) neuropeptide family that is selectively bound  by type 2 CRF receptors.	bind
49925	2	10886	5	13	NULL	NULL	NULL	type 2 CRF receptors	GP		bind		selectively			member of CRF neuropeptide family	GP				NULL		NULL	NULL	NULL	NULL	gw70_brainres_980_2_206_s_337	12867260	A member of the  corticotropin-releasing factor (CRF) neuropeptide family that is selectively bound  by type 2 CRF receptors.	bind
41920	1	10886	6	NULL	NULL	0	NULL	CRF	NULL		is	NULL				corticotropin-releasing factor	NULL				NULL		0	NULL	NULL	NULL	gw70_brainres_980_2_206_s_337	12867260	A member of the  corticotropin-releasing factor (CRF) neuropeptide family that is selectively bound  by type 2 CRF receptors.	bind
41921	2	10886	6	NULL	NULL	0	NULL	member of CRF family	NULL		bind	NULL	selectively			type 2 CRF receptors	NULL				NULL		0	NULL	NULL	NULL	gw70_brainres_980_2_206_s_337	12867260	A member of the  corticotropin-releasing factor (CRF) neuropeptide family that is selectively bound  by type 2 CRF receptors.	bind
49926	1	10889	5	13	NULL	NULL	NULL	Meis1 homeodomain family member	GP		bind					CRS1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_14_7941_s_86	9525891	A member of the Meis1 homeodomain family binds CRS1.	bind
41922	1	10889	6	NULL	NULL	0	NULL	Meis1 homeodomain family member	NULL		bind	NULL				CRS1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_7941_s_86	9525891	A member of the Meis1 homeodomain family binds CRS1.	bind
49927	1	10890	5	13	NULL	NULL	NULL	AR	GP		is a member of					steroid hormone receptor family	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_45_37853_s_12	16141201	A member of the steroid hormone receptor family, AR binds androgen and drives the transcription of androgen-responsive genes in a variety of tissues and cell types.	bind
49928	2	10890	5	13	NULL	NULL	NULL	AR	GP		bind					androgen	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_45_37853_s_12	16141201	A member of the steroid hormone receptor family, AR binds androgen and drives the transcription of androgen-responsive genes in a variety of tissues and cell types.	bind
49929	3	10890	5	13	NULL	NULL	NULL	statement 2	Process		drives					androgen-responsive genes	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_45_37853_s_12	16141201	A member of the steroid hormone receptor family, AR binds androgen and drives the transcription of androgen-responsive genes in a variety of tissues and cell types.	bind
41923	1	10890	6	NULL	NULL	0	NULL	AR	NULL		bind	NULL				androgen	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_45_37853_s_12	16141201	A member of the steroid hormone receptor family, AR binds androgen and drives the transcription of androgen-responsive genes in a variety of tissues and cell types.	bind
41924	2	10890	6	10	NULL	0	NULL	AR	NULL		is a member of	NULL				steroid hormone receptor family	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_45_37853_s_12	16141201	A member of the steroid hormone receptor family, AR binds androgen and drives the transcription of androgen-responsive genes in a variety of tissues and cell types.	bind
41925	3	10890	6	NULL	NULL	0	NULL	statement 1	NULL		drives	NULL				androgen responsive genes	NULL	transcription of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_45_37853_s_12	16141201	A member of the steroid hormone receptor family, AR binds androgen and drives the transcription of androgen-responsive genes in a variety of tissues and cell types.	bind
49930	1	10892	5	13	NULL	NULL	NULL	photoreceptor apoprotein	GP		bind		reversibly			riboflavin	Chemical	free			NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiolrev_25_5_503_s_203	11742688	A membrane protein that binds free riboflavin reversibly is a plausible photoreceptor apoprotein [  31].	bind
49931	2	10892	5	13	NULL	NULL	NULL	photoreceptor apoprotein	GP		is a type of					membrane protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiolrev_25_5_503_s_203	11742688	A membrane protein that binds free riboflavin reversibly is a plausible photoreceptor apoprotein [  31].	bind
41926	1	10892	6	NULL	NULL	0	NULL	photoreceptor apoprotein	NULL		bind	NULL	reversibly			riboflavin	NULL	free			NULL		0	NULL	NULL	NULL	gw60_femsmicrobiolrev_25_5_503_s_203	11742688	A membrane protein that binds free riboflavin reversibly is a plausible photoreceptor apoprotein [  31].	bind
41927	2	10892	6	NULL	NULL	0	NULL	photoreceptor apoprotein	NULL		is a type of	NULL				membrane protein	NULL				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiolrev_25_5_503_s_203	11742688	A membrane protein that binds free riboflavin reversibly is a plausible photoreceptor apoprotein [  31].	bind
49932	1	10893	5	13	NULL	NULL	NULL	E-cadherin protein	GP		bind					C3G	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_15_6690_s_57	15254236	A membrane was incubated with 200 nM GST-E-cadherin, and the E-cadherin protein bound to C3G on the membrane was detected by anti-E-cadherin antibody.	bind
41928	1	10893	6	NULL	NULL	0	NULL	E-cadherin protein	NULL		bind	NULL				C3G	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_15_6690_s_57	15254236	A membrane was incubated with 200 nM GST-E-cadherin, and the E-cadherin protein bound to C3G on the membrane was detected by anti-E-cadherin antibody.	bind
49933	1	10894	5	13	NULL	NULL	NULL	minireceptor	GP	membrane-anchored	does not bind					alpha2M	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_11_6057_s_236	9497322	A membrane-anchored minireceptor that contained all eight class A repeats of cluster II but not the neighboring fourth epidermal growth factor repeat did not show binding to alpha2M ( 11).	bind
49934	2	10894	5	13	NULL	NULL	NULL	minireceptor	GP	membrane-anchored	contains								class A repeats of cluster II		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_11_6057_s_236	9497322	A membrane-anchored minireceptor that contained all eight class A repeats of cluster II but not the neighboring fourth epidermal growth factor repeat did not show binding to alpha2M ( 11).	bind
49935	3	10894	5	13	NULL	NULL	NULL	minireceptor	GP	membrane-anchored	does not contain								fourth epidermal growth factor repeat		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_11_6057_s_236	9497322	A membrane-anchored minireceptor that contained all eight class A repeats of cluster II but not the neighboring fourth epidermal growth factor repeat did not show binding to alpha2M ( 11).	bind
42059	1	10894	6	NULL	NULL	0	NULL	minireceptor	NULL	membrane-anchored	contains	NULL					NULL		class A repeats of cluster II		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_11_6057_s_236	9497322	A membrane-anchored minireceptor that contained all eight class A repeats of cluster II but not the neighboring fourth epidermal growth factor repeat did not show binding to alpha2M ( 11).	bind
42060	2	10894	6	NULL	NULL	0	NULL	statement 1	NULL		does not bind	NULL				alpha2M	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_11_6057_s_236	9497322	A membrane-anchored minireceptor that contained all eight class A repeats of cluster II but not the neighboring fourth epidermal growth factor repeat did not show binding to alpha2M ( 11).	bind
42061	3	10894	6	NULL	NULL	0	NULL	minireceptor	NULL	membrane-anchored	does not contain	NULL					NULL		fourth epidermal growth factor repeat		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_11_6057_s_236	9497322	A membrane-anchored minireceptor that contained all eight class A repeats of cluster II but not the neighboring fourth epidermal growth factor repeat did not show binding to alpha2M ( 11).	bind
49936	1	10895	5	13	NULL	NULL	NULL	AZ-521	Cell		is a type of					human gastric cancer cell lines	Cell				NULL		NULL	NULL	NULL	NULL	gw60_annurevmicrobiol_53_0_353_s_176	10547695	A membrane-bound 140-kDa   protein present in human gastric cancer cell lines (AZ-521 and AGS)   has been identified as a potential receptor for binding of VacA to   target cells because this protein was coimmunoprecipitated with   VacA by anti-VacA antibodies ( 177).	bind
49937	2	10895	5	13	NULL	NULL	NULL	AGS	Cell		is a type of					human gastric cancer cell lines	Cell				NULL		NULL	NULL	NULL	NULL	gw60_annurevmicrobiol_53_0_353_s_176	10547695	A membrane-bound 140-kDa   protein present in human gastric cancer cell lines (AZ-521 and AGS)   has been identified as a potential receptor for binding of VacA to   target cells because this protein was coimmunoprecipitated with   VacA by anti-VacA antibodies ( 177).	bind
49938	3	10895	5	13	NULL	NULL	NULL	VacA	GP		bind					target cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_annurevmicrobiol_53_0_353_s_176	10547695	A membrane-bound 140-kDa   protein present in human gastric cancer cell lines (AZ-521 and AGS)   has been identified as a potential receptor for binding of VacA to   target cells because this protein was coimmunoprecipitated with   VacA by anti-VacA antibodies ( 177).	bind
49939	5	10895	5	13	NULL	NULL	NULL	statement 4	GP		is a receptor for		potentially			statement 3	GP				NULL		NULL	NULL	NULL	NULL	gw60_annurevmicrobiol_53_0_353_s_176	10547695	A membrane-bound 140-kDa   protein present in human gastric cancer cell lines (AZ-521 and AGS)   has been identified as a potential receptor for binding of VacA to   target cells because this protein was coimmunoprecipitated with   VacA by anti-VacA antibodies ( 177).	bind
49940	6	10895	5	13	NULL	NULL	NULL	statement 4	GP		is present in					AZ-521	Cell				NULL		NULL	NULL	NULL	NULL	gw60_annurevmicrobiol_53_0_353_s_176	10547695	A membrane-bound 140-kDa   protein present in human gastric cancer cell lines (AZ-521 and AGS)   has been identified as a potential receptor for binding of VacA to   target cells because this protein was coimmunoprecipitated with   VacA by anti-VacA antibodies ( 177).	bind
49941	7	10895	5	13	NULL	NULL	NULL	statement 4	GP		is present in					AGS	Cell				NULL		NULL	NULL	NULL	NULL	gw60_annurevmicrobiol_53_0_353_s_176	10547695	A membrane-bound 140-kDa   protein present in human gastric cancer cell lines (AZ-521 and AGS)   has been identified as a potential receptor for binding of VacA to   target cells because this protein was coimmunoprecipitated with   VacA by anti-VacA antibodies ( 177).	bind
50472	4	10895	5	13	NULL	NULL	NULL	140-kDa protein	GP		bind					membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_annurevmicrobiol_53_0_353_s_176	10547695	A membrane-bound 140-kDa   protein present in human gastric cancer cell lines (AZ-521 and AGS)   has been identified as a potential receptor for binding of VacA to   target cells because this protein was coimmunoprecipitated with   VacA by anti-VacA antibodies ( 177).	bind
41929	1	10895	6	NULL	NULL	0	NULL	AZ-521	NULL		is a type of	NULL				gastric cancer cell line	NULL	human			NULL		0	NULL	NULL	NULL	gw60_annurevmicrobiol_53_0_353_s_176	10547695	A membrane-bound 140-kDa   protein present in human gastric cancer cell lines (AZ-521 and AGS)   has been identified as a potential receptor for binding of VacA to   target cells because this protein was coimmunoprecipitated with   VacA by anti-VacA antibodies ( 177).	bind
41930	2	10895	6	NULL	NULL	0	NULL	AGS	NULL		is a type of	NULL				gastric cancer cell line	NULL	human			NULL		0	NULL	NULL	NULL	gw60_annurevmicrobiol_53_0_353_s_176	10547695	A membrane-bound 140-kDa   protein present in human gastric cancer cell lines (AZ-521 and AGS)   has been identified as a potential receptor for binding of VacA to   target cells because this protein was coimmunoprecipitated with   VacA by anti-VacA antibodies ( 177).	bind
41931	3	10895	6	NULL	NULL	0	NULL	VacA	NULL		bind	NULL				target cells	NULL				NULL		0	NULL	NULL	NULL	gw60_annurevmicrobiol_53_0_353_s_176	10547695	A membrane-bound 140-kDa   protein present in human gastric cancer cell lines (AZ-521 and AGS)   has been identified as a potential receptor for binding of VacA to   target cells because this protein was coimmunoprecipitated with   VacA by anti-VacA antibodies ( 177).	bind
41932	5	10895	6	10	NULL	0	NULL	statement 4	NULL		acts as a receptor for	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_annurevmicrobiol_53_0_353_s_176	10547695	A membrane-bound 140-kDa   protein present in human gastric cancer cell lines (AZ-521 and AGS)   has been identified as a potential receptor for binding of VacA to   target cells because this protein was coimmunoprecipitated with   VacA by anti-VacA antibodies ( 177).	bind
41933	6	10895	6	10	NULL	0	NULL	statement 4	NULL		is present in	NULL				AZ-521	NULL				NULL		NULL	NULL	NULL	NULL	gw60_annurevmicrobiol_53_0_353_s_176	10547695	A membrane-bound 140-kDa   protein present in human gastric cancer cell lines (AZ-521 and AGS)   has been identified as a potential receptor for binding of VacA to   target cells because this protein was coimmunoprecipitated with   VacA by anti-VacA antibodies ( 177).	bind
41934	7	10895	6	10	NULL	0	NULL	statement 4	NULL		is present in	NULL				AGS	NULL				NULL		NULL	NULL	NULL	NULL	gw60_annurevmicrobiol_53_0_353_s_176	10547695	A membrane-bound 140-kDa   protein present in human gastric cancer cell lines (AZ-521 and AGS)   has been identified as a potential receptor for binding of VacA to   target cells because this protein was coimmunoprecipitated with   VacA by anti-VacA antibodies ( 177).	bind
50473	4	10895	6	10	NULL	0	NULL	140-kDa protein	NULL		bind	NULL				membrane	NULL				NULL		0	NULL	NULL	NULL	gw60_annurevmicrobiol_53_0_353_s_176	10547695	A membrane-bound 140-kDa   protein present in human gastric cancer cell lines (AZ-521 and AGS)   has been identified as a potential receptor for binding of VacA to   target cells because this protein was coimmunoprecipitated with   VacA by anti-VacA antibodies ( 177).	bind
49943	2	10897	5	13	NULL	NULL	NULL	metabolite of acetaminophen	Chemical		bind		covalently			56 kDa selenium binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_280_1_501_s_255	8996234	A metabolite of acetaminophen covalently binds to the 56 kDa selenium binding protein.	bind
41935	1	10897	6	NULL	NULL	0	NULL	acetaminophen metabolite	NULL		bind	NULL	covalently			56 kDa selenium binding protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_280_1_501_s_255	8996234	A metabolite of acetaminophen covalently binds to the 56 kDa selenium binding protein.	bind
49944	1	10898	5	13	NULL	NULL	NULL	VEGF	GP		bind					VEGF receptor	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_arch-pharm-res_28_11_16350854_s_4	16350854	A methanol extract and organic solvent (n-hexane,  ethyl acetate, n-butanol, aqueous) fractions from Rubus coreanus were  examined for their inhibitory effects on VEGF binding to the VEGF receptor.	bind
41936	1	10898	6	NULL	NULL	0	NULL	VEGF	NULL		bind	NULL				VEGF receptor	NULL				NULL		0	NULL	NULL	NULL	abs-batch0550-0559_arch-pharm-res_28_11_16350854_s_4	16350854	A methanol extract and organic solvent (n-hexane,  ethyl acetate, n-butanol, aqueous) fractions from Rubus coreanus were  examined for their inhibitory effects on VEGF binding to the VEGF receptor.	bind
49945	1	10900	5	13	NULL	NULL	NULL	antimycin A	Chemical	methoxy derivative of 	bind					Bcl-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_115_10_2648_s_174	16200198	A methoxy derivative of antimycin A binds to Bcl-2 with a  Kd of 0.82 muM ( ).	bind
41937	1	10900	6	10	NULL	0	NULL	antimycin A 	NULL	methoxy derivative of 	bind	NULL				Bcl-2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_115_10_2648_s_174	16200198	A methoxy derivative of antimycin A binds to Bcl-2 with a  Kd of 0.82 muM ( ).	bind
49946	1	10901	5	13	NULL	NULL	NULL	copper transport proteins	GP		bind		selectively	Mets motif peptide		Cu(I)	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_inorg-chem_44_26_16363848_s_1	16363848	A Mets motif peptide found in copper transport proteins selectively binds Cu(I) with methionine-only coordination..	bind
41938	1	10901	6	NULL	NULL	0	NULL	copper transport protein	NULL		bind	NULL	selectively	Mets motif peptide		Cu(I)	NULL				NULL		0	NULL	NULL	NULL	abs-batch0550-0559_inorg-chem_44_26_16363848_s_1	16363848	A Mets motif peptide found in copper transport proteins selectively binds Cu(I) with methionine-only coordination..	bind
49947	1	10902	5	13	NULL	NULL	NULL	GTP	Chemical	non-exchangeable	bind								alpha-subunit		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33803_s_14	9837970	A Mg2+ ion coordinated with non-exchangeable GTP bound to the alpha-subunit near the alpha-beta dimerization interface controls the stability of the heterodimer ( 1), whereas the cation and exchangeable nucleotide bound to the beta-subunit, near the beta-alpha axial interface leading to protofilament formation ( 2) control microtubule stability.	bind
49948	2	10902	5	13	NULL	NULL	NULL	Mg2+ ion	Chemical		coordinates with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33803_s_14	9837970	A Mg2+ ion coordinated with non-exchangeable GTP bound to the alpha-subunit near the alpha-beta dimerization interface controls the stability of the heterodimer ( 1), whereas the cation and exchangeable nucleotide bound to the beta-subunit, near the beta-alpha axial interface leading to protofilament formation ( 2) control microtubule stability.	bind
49949	3	10902	5	13	NULL	NULL	NULL	statement 2	Process		is located near								alpha-beta dimerization interface		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33803_s_14	9837970	A Mg2+ ion coordinated with non-exchangeable GTP bound to the alpha-subunit near the alpha-beta dimerization interface controls the stability of the heterodimer ( 1), whereas the cation and exchangeable nucleotide bound to the beta-subunit, near the beta-alpha axial interface leading to protofilament formation ( 2) control microtubule stability.	bind
49950	4	10902	5	13	NULL	NULL	NULL	statement 2	Process		controls					statement 1	Process	stability of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33803_s_14	9837970	A Mg2+ ion coordinated with non-exchangeable GTP bound to the alpha-subunit near the alpha-beta dimerization interface controls the stability of the heterodimer ( 1), whereas the cation and exchangeable nucleotide bound to the beta-subunit, near the beta-alpha axial interface leading to protofilament formation ( 2) control microtubule stability.	bind
49951	5	10902	5	13	NULL	NULL	NULL	cation	Chemical		bind								beta-subunit		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33803_s_14	9837970	A Mg2+ ion coordinated with non-exchangeable GTP bound to the alpha-subunit near the alpha-beta dimerization interface controls the stability of the heterodimer ( 1), whereas the cation and exchangeable nucleotide bound to the beta-subunit, near the beta-alpha axial interface leading to protofilament formation ( 2) control microtubule stability.	bind
49952	6	10902	5	13	NULL	NULL	NULL	statement 5	Process		is located near								beta-alpha axial interface		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33803_s_14	9837970	A Mg2+ ion coordinated with non-exchangeable GTP bound to the alpha-subunit near the alpha-beta dimerization interface controls the stability of the heterodimer ( 1), whereas the cation and exchangeable nucleotide bound to the beta-subunit, near the beta-alpha axial interface leading to protofilament formation ( 2) control microtubule stability.	bind
49953	7	10902	5	13	NULL	NULL	NULL	statement 5	Process		leads to					protofilament	CellComponent	formation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33803_s_14	9837970	A Mg2+ ion coordinated with non-exchangeable GTP bound to the alpha-subunit near the alpha-beta dimerization interface controls the stability of the heterodimer ( 1), whereas the cation and exchangeable nucleotide bound to the beta-subunit, near the beta-alpha axial interface leading to protofilament formation ( 2) control microtubule stability.	bind
49954	8	10902	5	13	NULL	NULL	NULL	nucleotide	NucleicAcid	exchangeable	bind								beta-subunit		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33803_s_14	9837970	A Mg2+ ion coordinated with non-exchangeable GTP bound to the alpha-subunit near the alpha-beta dimerization interface controls the stability of the heterodimer ( 1), whereas the cation and exchangeable nucleotide bound to the beta-subunit, near the beta-alpha axial interface leading to protofilament formation ( 2) control microtubule stability.	bind
49955	9	10902	5	13	NULL	NULL	NULL	statement 8	Process		is located near								beta-alpha axial interface		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33803_s_14	9837970	A Mg2+ ion coordinated with non-exchangeable GTP bound to the alpha-subunit near the alpha-beta dimerization interface controls the stability of the heterodimer ( 1), whereas the cation and exchangeable nucleotide bound to the beta-subunit, near the beta-alpha axial interface leading to protofilament formation ( 2) control microtubule stability.	bind
49956	10	10902	5	13	NULL	NULL	NULL	statement 8	Process		leads to					protofilament	CellComponent	formation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33803_s_14	9837970	A Mg2+ ion coordinated with non-exchangeable GTP bound to the alpha-subunit near the alpha-beta dimerization interface controls the stability of the heterodimer ( 1), whereas the cation and exchangeable nucleotide bound to the beta-subunit, near the beta-alpha axial interface leading to protofilament formation ( 2) control microtubule stability.	bind
49957	11	10902	5	13	NULL	NULL	NULL	statement 5	Process		controls					microtubule	CellComponent	stability of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33803_s_14	9837970	A Mg2+ ion coordinated with non-exchangeable GTP bound to the alpha-subunit near the alpha-beta dimerization interface controls the stability of the heterodimer ( 1), whereas the cation and exchangeable nucleotide bound to the beta-subunit, near the beta-alpha axial interface leading to protofilament formation ( 2) control microtubule stability.	bind
49958	12	10902	5	13	NULL	NULL	NULL	statement 8	Process		controls					microtubule 	CellComponent	stability of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33803_s_14	9837970	A Mg2+ ion coordinated with non-exchangeable GTP bound to the alpha-subunit near the alpha-beta dimerization interface controls the stability of the heterodimer ( 1), whereas the cation and exchangeable nucleotide bound to the beta-subunit, near the beta-alpha axial interface leading to protofilament formation ( 2) control microtubule stability.	bind
42062	1	10902	6	10	NULL	0	NULL	GTP		non-exchangeable	bind								alpha-subunit		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33803_s_14	9837970	A Mg2+ ion coordinated with non-exchangeable GTP bound to the alpha-subunit near the alpha-beta dimerization interface controls the stability of the heterodimer ( 1), whereas the cation and exchangeable nucleotide bound to the beta-subunit, near the beta-alpha axial interface leading to protofilament formation ( 2) control microtubule stability.	bind
42063	2	10902	6	10	NULL	0	NULL	Mg2+ ion			is coordinated with					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33803_s_14	9837970	A Mg2+ ion coordinated with non-exchangeable GTP bound to the alpha-subunit near the alpha-beta dimerization interface controls the stability of the heterodimer ( 1), whereas the cation and exchangeable nucleotide bound to the beta-subunit, near the beta-alpha axial interface leading to protofilament formation ( 2) control microtubule stability.	bind
42064	3	10902	6	10	NULL	0	NULL	statement 1			controls					statement 1		stability of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33803_s_14	9837970	A Mg2+ ion coordinated with non-exchangeable GTP bound to the alpha-subunit near the alpha-beta dimerization interface controls the stability of the heterodimer ( 1), whereas the cation and exchangeable nucleotide bound to the beta-subunit, near the beta-alpha axial interface leading to protofilament formation ( 2) control microtubule stability.	bind
50816	4	10902	6	NULL	NULL	0	NULL	statement 2	NULL		occurs near	NULL				alpha-beta dimerization interface	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_50_33803_s_14	9837970	A Mg2+ ion coordinated with non-exchangeable GTP bound to the alpha-subunit near the alpha-beta dimerization interface controls the stability of the heterodimer ( 1), whereas the cation and exchangeable nucleotide bound to the beta-subunit, near the beta-alpha axial interface leading to protofilament formation ( 2) control microtubule stability.	bind
50817	5	10902	6	NULL	NULL	0	NULL	beta-subunit	NULL		bind	NULL				nucleotide	NULL	exchangeable			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33803_s_14	9837970	A Mg2+ ion coordinated with non-exchangeable GTP bound to the alpha-subunit near the alpha-beta dimerization interface controls the stability of the heterodimer ( 1), whereas the cation and exchangeable nucleotide bound to the beta-subunit, near the beta-alpha axial interface leading to protofilament formation ( 2) control microtubule stability.	bind
50818	6	10902	6	NULL	NULL	0	NULL	cation	NULL		bind	NULL				beta-subunit	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_50_33803_s_14	9837970	A Mg2+ ion coordinated with non-exchangeable GTP bound to the alpha-subunit near the alpha-beta dimerization interface controls the stability of the heterodimer ( 1), whereas the cation and exchangeable nucleotide bound to the beta-subunit, near the beta-alpha axial interface leading to protofilament formation ( 2) control microtubule stability.	bind
50819	7	10902	6	NULL	NULL	0	NULL	statement 5	NULL		leads to	NULL				protofilament 	NULL	formation of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_50_33803_s_14	9837970	A Mg2+ ion coordinated with non-exchangeable GTP bound to the alpha-subunit near the alpha-beta dimerization interface controls the stability of the heterodimer ( 1), whereas the cation and exchangeable nucleotide bound to the beta-subunit, near the beta-alpha axial interface leading to protofilament formation ( 2) control microtubule stability.	bind
50820	8	10902	6	NULL	NULL	0	NULL	statement 6	NULL		leads to	NULL				protofilament	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_50_33803_s_14	9837970	A Mg2+ ion coordinated with non-exchangeable GTP bound to the alpha-subunit near the alpha-beta dimerization interface controls the stability of the heterodimer ( 1), whereas the cation and exchangeable nucleotide bound to the beta-subunit, near the beta-alpha axial interface leading to protofilament formation ( 2) control microtubule stability.	bind
50821	9	10902	6	NULL	NULL	0	NULL	statement 5	NULL		occurs near	NULL				beta-alpha axial interface	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33803_s_14	9837970	A Mg2+ ion coordinated with non-exchangeable GTP bound to the alpha-subunit near the alpha-beta dimerization interface controls the stability of the heterodimer ( 1), whereas the cation and exchangeable nucleotide bound to the beta-subunit, near the beta-alpha axial interface leading to protofilament formation ( 2) control microtubule stability.	bind
50822	10	10902	6	NULL	NULL	0	NULL	statement 6	NULL		occurs near	NULL				beta-alpha axial interface	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_50_33803_s_14	9837970	A Mg2+ ion coordinated with non-exchangeable GTP bound to the alpha-subunit near the alpha-beta dimerization interface controls the stability of the heterodimer ( 1), whereas the cation and exchangeable nucleotide bound to the beta-subunit, near the beta-alpha axial interface leading to protofilament formation ( 2) control microtubule stability.	bind
58413	11	10902	6	10	NULL	0	NULL	statement 5			controls					microtubule		stability of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_50_33803_s_14	9837970	A Mg2+ ion coordinated with non-exchangeable GTP bound to the alpha-subunit near the alpha-beta dimerization interface controls the stability of the heterodimer ( 1), whereas the cation and exchangeable nucleotide bound to the beta-subunit, near the beta-alpha axial interface leading to protofilament formation ( 2) control microtubule stability.	bind
58414	12	10902	6	10	NULL	0	NULL	statement 6			controls					microtubule		stability of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_50_33803_s_14	9837970	A Mg2+ ion coordinated with non-exchangeable GTP bound to the alpha-subunit near the alpha-beta dimerization interface controls the stability of the heterodimer ( 1), whereas the cation and exchangeable nucleotide bound to the beta-subunit, near the beta-alpha axial interface leading to protofilament formation ( 2) control microtubule stability.	bind
49959	1	10903	5	13	NULL	NULL	NULL	FAT10	GP		is a type of					MHC-encoded ubiquitin-like protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_18_5509_s_431	9312010	A MHC-encoded ubiquitin-like protein (FAT10) binds noncovalently to the spindle assembly checkpoint protein MAD2.	bind
49960	2	10903	5	13	NULL	NULL	NULL	MAD2	GP		is a type of					spindle assembly checkpoint protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_18_5509_s_431	9312010	A MHC-encoded ubiquitin-like protein (FAT10) binds noncovalently to the spindle assembly checkpoint protein MAD2.	bind
49961	3	10903	5	13	NULL	NULL	NULL	FAT10	GP		bind		noncovalently			MAD2	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_18_5509_s_431	9312010	A MHC-encoded ubiquitin-like protein (FAT10) binds noncovalently to the spindle assembly checkpoint protein MAD2.	bind
41939	1	10903	6	NULL	NULL	0	NULL	FAT10	NULL		is a type of	NULL				MHC-encoded ubiquitin-like protein	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_16_18_5509_s_431	9312010	A MHC-encoded ubiquitin-like protein (FAT10) binds noncovalently to the spindle assembly checkpoint protein MAD2.	bind
41940	2	10903	6	NULL	NULL	0	NULL	MAD2	NULL		is a type of	NULL				spindle assembly checkpoint protein	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_16_18_5509_s_431	9312010	A MHC-encoded ubiquitin-like protein (FAT10) binds noncovalently to the spindle assembly checkpoint protein MAD2.	bind
41941	3	10903	6	NULL	NULL	0	NULL	FAT10	NULL		bind	NULL	noncovalently			MAD2	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_16_18_5509_s_431	9312010	A MHC-encoded ubiquitin-like protein (FAT10) binds noncovalently to the spindle assembly checkpoint protein MAD2.	bind
50474	1	10905	5	13	NULL	NULL	NULL	IscU	GP		bind					Hsc20	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_14_7790_s_63	10869428	A Microcal (Amherst, MA) Omega titration calorimeter was used to investigate the binding of IscU and Hsc20 by using procedures described previously ( 27).	bind
41942	1	10905	6	NULL	NULL	0	NULL	IScU	NULL		bind	NULL				Hsc20	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_14_7790_s_63	10869428	A Microcal (Amherst, MA) Omega titration calorimeter was used to investigate the binding of IscU and Hsc20 by using procedures described previously ( 27).	bind
50476	1	10906	5	13	NULL	NULL	NULL	IscU protein	GP		bind					Hsc66	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_39_37582_s_63	12871959	A Microcal Omega microcalorimeter (Amherst, MA) was used to investigate the binding of IscU proteins to Hsc66 and Hsc20.	bind
50477	2	10906	5	13	NULL	NULL	NULL	IscU protein	GP		bind					Hsc20	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_39_37582_s_63	12871959	A Microcal Omega microcalorimeter (Amherst, MA) was used to investigate the binding of IscU proteins to Hsc66 and Hsc20.	bind
41945	2	10906	6	NULL	NULL	0	NULL	IscU protein	NULL		bind	NULL				Hsc20	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_39_37582_s_63	12871959	A Microcal Omega microcalorimeter (Amherst, MA) was used to investigate the binding of IscU proteins to Hsc66 and Hsc20.	bind
50475	1	10906	6	10	NULL	0	NULL	IscU protein	NULL		bind	NULL				Hsc66	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_39_37582_s_63	12871959	A Microcal Omega microcalorimeter (Amherst, MA) was used to investigate the binding of IscU proteins to Hsc66 and Hsc20.	bind
49962	1	10907	5	13	NULL	NULL	NULL	GtfI	GP		bind			GBD		alpha-1,3 glucan	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_24_8301_s_7	15576779	A microplate binding assay was developed to measure the binding affinity of recombinant GBDs. GBD of GtfI was shown to be capable of binding glucans with predominantly alpha-1,3 or alpha-1,6 links, as well as alternating alpha-1,3 and alpha-1,6 links (alternan).	bind
49963	2	10907	5	13	NULL	NULL	NULL	GtfI	GP		bind			GBD		alpha-1,6 glucan	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_24_8301_s_7	15576779	A microplate binding assay was developed to measure the binding affinity of recombinant GBDs. GBD of GtfI was shown to be capable of binding glucans with predominantly alpha-1,3 or alpha-1,6 links, as well as alternating alpha-1,3 and alpha-1,6 links (alternan).	bind
42065	1	10907	6	NULL	NULL	0	NULL	GtfI	NULL		bind	NULL	predominantly	GBD		alpha-1,3-glucans	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_24_8301_s_7	15576779	A microplate binding assay was developed to measure the binding affinity of recombinant GBDs. GBD of GtfI was shown to be capable of binding glucans with predominantly alpha-1,3 or alpha-1,6 links, as well as alternating alpha-1,3 and alpha-1,6 links (alternan).	bind
42066	2	10907	6	NULL	NULL	0	NULL	GtfI	NULL		bind	NULL	predominantly	GBD		alpha-1,6 glucan	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_24_8301_s_7	15576779	A microplate binding assay was developed to measure the binding affinity of recombinant GBDs. GBD of GtfI was shown to be capable of binding glucans with predominantly alpha-1,3 or alpha-1,6 links, as well as alternating alpha-1,3 and alpha-1,6 links (alternan).	bind
49964	1	10911	5	13	NULL	NULL	NULL				shows			G519A		peripheral accumulation	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1506_s_111	15014437	A milder mutation at G519 (G519A rather than G519R) showed peripheral accumulation  and MT binding similar to that of G519R (data not shown).	bind
49965	2	10911	5	13	NULL	NULL	NULL				bind			G519A		MT	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1506_s_111	15014437	A milder mutation at G519 (G519A rather than G519R) showed peripheral accumulation  and MT binding similar to that of G519R (data not shown).	bind
49966	3	10911	5	13	NULL	NULL	NULL				shows			G519R		peripheral accumulation	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1506_s_111	15014437	A milder mutation at G519 (G519A rather than G519R) showed peripheral accumulation  and MT binding similar to that of G519R (data not shown).	bind
49967	4	10911	5	13	NULL	NULL	NULL				bind			G519R		MT	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1506_s_111	15014437	A milder mutation at G519 (G519A rather than G519R) showed peripheral accumulation  and MT binding similar to that of G519R (data not shown).	bind
41946	1	10911	6	NULL	NULL	0	NULL		NULL		bind	NULL		G519A		MT	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_23_7_1506_s_111	15014437	A milder mutation at G519 (G519A rather than G519R) showed peripheral accumulation  and MT binding similar to that of G519R (data not shown).	bind
41947	2	10911	6	NULL	NULL	0	NULL		NULL		shows	NULL		G519A		peripheral accumulation	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_23_7_1506_s_111	15014437	A milder mutation at G519 (G519A rather than G519R) showed peripheral accumulation  and MT binding similar to that of G519R (data not shown).	bind
41948	3	10911	6	NULL	NULL	0	NULL		NULL		bind	NULL		G519R		MT	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_23_7_1506_s_111	15014437	A milder mutation at G519 (G519A rather than G519R) showed peripheral accumulation  and MT binding similar to that of G519R (data not shown).	bind
41949	4	10911	6	NULL	NULL	0	NULL		NULL		shows	NULL		G519R		peripheral accumulation	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_23_7_1506_s_111	15014437	A milder mutation at G519 (G519A rather than G519R) showed peripheral accumulation  and MT binding similar to that of G519R (data not shown).	bind
49968	1	10912	5	13	NULL	NULL	NULL	tRNAiMet	NucleicAcid	yeast	forms complex with		stably	acceptor stem		LysRS	GP	mammalian			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_1762_s_175	11706011	A minihelix corresponding to a noncognate tRNA, the acceptor stem of yeast tRNAiMet, also formed a stable complex with LysRS with an apparent  K d of 1 muM (not shown), further exemplifying the general RNA binding potency of mammalian LysRS.	bind
42067	1	10912	6	10	NULL	0	NULL	tRNAiMet	NULL	yeast	forms a complex with	NULL	stably	acceptor stem		LysRS	NULL	mammalian			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_1762_s_175	11706011	A minihelix corresponding to a noncognate tRNA, the acceptor stem of yeast tRNAiMet, also formed a stable complex with LysRS with an apparent  K d of 1 muM (not shown), further exemplifying the general RNA binding potency of mammalian LysRS.	bind
49969	1	10913	5	13	NULL	NULL	NULL	Dal80p dimer	GP		bind		may			DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_21_5682_s_4	9791119	A minimal Gln3p binding site consists of a single GATA sequence, whereas a Dal80p binding site consists of two GATA sequences in specific orientation, 15 to 35 bp apart, suggesting that Dal80p may bind to DNA as a dimer.	bind
50478	2	10913	5	13	NULL	NULL	NULL	Dal80p	GP		consist of				binding site					two GATA sequences	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_21_5682_s_4	9791119	A minimal Gln3p binding site consists of a single GATA sequence, whereas a Dal80p binding site consists of two GATA sequences in specific orientation, 15 to 35 bp apart, suggesting that Dal80p may bind to DNA as a dimer.	bind
41950	1	10913	6	10	NULL	0	NULL	Dal80p dimer	NULL		bind	NULL	may			DNA	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_21_5682_s_4	9791119	A minimal Gln3p binding site consists of a single GATA sequence, whereas a Dal80p binding site consists of two GATA sequences in specific orientation, 15 to 35 bp apart, suggesting that Dal80p may bind to DNA as a dimer.	bind
50479	2	10913	6	10	NULL	0	NULL	Dal80p	NULL		consist of	NULL			binding site		NULL			two GATA sequences	NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_21_5682_s_4	9791119	A minimal Gln3p binding site consists of a single GATA sequence, whereas a Dal80p binding site consists of two GATA sequences in specific orientation, 15 to 35 bp apart, suggesting that Dal80p may bind to DNA as a dimer.	bind
49970	1	10914	5	13	NULL	NULL	NULL	ATP	Chemical		bind					ArsA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_23_16153_s_98	10347168	A minimal value can be calculated for the second-order association rate constant for the binding of ATP to the ArsA from ( kmax +  kmin)/ K d, yielding a value of 0.34 x 106M 1 s 1.	bind
41951	1	10914	6	NULL	NULL	0	NULL	ATP	NULL		bind	NULL				ArsA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_23_16153_s_98	10347168	A minimal value can be calculated for the second-order association rate constant for the binding of ATP to the ArsA from ( kmax +  kmin)/ K d, yielding a value of 0.34 x 106M 1 s 1.	bind
49971	1	10915	5	13	NULL	NULL	NULL	C3d	GP		enhances			CR2 binding domain		immunity	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_adv-exp-med-biol_586_1_16893077_s_1	16893077	A minimum CR2 binding domain of C3d enhances immunity following vaccination..	bind
49972	2	10915	5	13	NULL	NULL	NULL	statement 1	Process		occurs following					vaccination	MedicalProcedure				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_adv-exp-med-biol_586_1_16893077_s_1	16893077	A minimum CR2 binding domain of C3d enhances immunity following vaccination..	bind
41952	1	10915	6	NULL	NULL	0	NULL	C3d	NULL		enhances	NULL		CR2 binding domain		immunity	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_adv-exp-med-biol_586_1_16893077_s_1	16893077	A minimum CR2 binding domain of C3d enhances immunity following vaccination..	bind
49973	1	10918	5	13	NULL	NULL	NULL	heparin	Chemical		bind					PF4	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevmed_50_0_129_s_85	10073268	A minimum of 12 saccharide units ( 28), a minimum degree of sulfation ( 16,  29), and an optimal binding ratio of heparin and PF4 are required to form the HIT antigen  ( 30).	bind
41954	1	10918	6	NULL	NULL	0	NULL	heparin	NULL		bind	NULL				PF4	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevmed_50_0_129_s_85	10073268	A minimum of 12 saccharide units ( 28), a minimum degree of sulfation ( 16,  29), and an optimal binding ratio of heparin and PF4 are required to form the HIT antigen  ( 30).	bind
49974	1	10919	5	13	NULL	NULL	NULL	proteins	GP		is expressed in					retina	OrganismPart	Drosophila			NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_15_0_231_s_377	10611962	A minimum of 13 proteins expressed in the Drosophila retina bind directly to calmodulin.	bind
49975	2	10919	5	13	NULL	NULL	NULL	statement 1	GP		bind		directly			calmodulin	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_15_0_231_s_377	10611962	A minimum of 13 proteins expressed in the Drosophila retina bind directly to calmodulin.	bind
41956	1	10919	6	NULL	NULL	0	NULL	proteins	NULL		expressed in	NULL				retina	NULL	Drosophila			NULL		0	NULL	NULL	NULL	gw70_annurevcelldevbiol_15_0_231_s_377	10611962	A minimum of 13 proteins expressed in the Drosophila retina bind directly to calmodulin.	bind
41957	2	10919	6	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL	directly			calmodulin	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevcelldevbiol_15_0_231_s_377	10611962	A minimum of 13 proteins expressed in the Drosophila retina bind directly to calmodulin.	bind
49976	1	10920	5	13	NULL	NULL	NULL	gp120JR-FL/CD4 complex	GP	soluble	bind					CCR5	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_11_5762_s_158	10823934	A minimum of two sulfotyrosines in positions 10 and 14 were required for efficient inhibition of soluble gp120JR-FL/CD4 complex binding to CCR5.	bind
49977	2	10920	5	13	NULL	NULL	NULL				inhibit		effectively	sulfotyrosines in positions 10 and 14		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_11_5762_s_158	10823934	A minimum of two sulfotyrosines in positions 10 and 14 were required for efficient inhibition of soluble gp120JR-FL/CD4 complex binding to CCR5.	bind
41958	1	10920	6	NULL	NULL	0	NULL	gp120JR-FL/CD4 complex	NULL	soluble	bind	NULL				CCR5	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_11_5762_s_158	10823934	A minimum of two sulfotyrosines in positions 10 and 14 were required for efficient inhibition of soluble gp120JR-FL/CD4 complex binding to CCR5.	bind
41959	2	10920	6	NULL	NULL	0	NULL		NULL		are required for	NULL		two sulfotyrosines in positions 10 and 14		statement 1	NULL	inhibiton of			NULL		0	NULL	NULL	NULL	gw60_pnas_97_11_5762_s_158	10823934	A minimum of two sulfotyrosines in positions 10 and 14 were required for efficient inhibition of soluble gp120JR-FL/CD4 complex binding to CCR5.	bind
49978	1	10921	5	13	NULL	NULL	NULL	NTPi	NucleicAcid		is					initiating nucleotide	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24991_s_173	16831816	A minimum requirement for  de novo initiation of RNA synthesis by BVDV and HCV RdRps involves binding of the initiating nucleotide (NTPi) to the P-site and binding of the first NTP substrate (NTPi+1) to the N-site.	bind
49979	2	10921	5	13	NULL	NULL	NULL	NTPi+1	Chemical		is					first NTP substrate	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24991_s_173	16831816	A minimum requirement for  de novo initiation of RNA synthesis by BVDV and HCV RdRps involves binding of the initiating nucleotide (NTPi) to the P-site and binding of the first NTP substrate (NTPi+1) to the N-site.	bind
49980	3	10921	5	13	NULL	NULL	NULL	NTPi	NucleicAcid		bind								P-site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24991_s_173	16831816	A minimum requirement for  de novo initiation of RNA synthesis by BVDV and HCV RdRps involves binding of the initiating nucleotide (NTPi) to the P-site and binding of the first NTP substrate (NTPi+1) to the N-site.	bind
49981	4	10921	5	13	NULL	NULL	NULL	NTPi+1	Chemical		bind								N-site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24991_s_173	16831816	A minimum requirement for  de novo initiation of RNA synthesis by BVDV and HCV RdRps involves binding of the initiating nucleotide (NTPi) to the P-site and binding of the first NTP substrate (NTPi+1) to the N-site.	bind
49982	5	10921	5	13	NULL	NULL	NULL	BVDV	Organism		initiates					RNA	NucleicAcid	de novo synthesis of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24991_s_173	16831816	A minimum requirement for  de novo initiation of RNA synthesis by BVDV and HCV RdRps involves binding of the initiating nucleotide (NTPi) to the P-site and binding of the first NTP substrate (NTPi+1) to the N-site.	bind
49983	6	10921	5	13	NULL	NULL	NULL	HCV RdRps	GP		initiates					RNA	NucleicAcid	de novo synthesis of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24991_s_173	16831816	A minimum requirement for  de novo initiation of RNA synthesis by BVDV and HCV RdRps involves binding of the initiating nucleotide (NTPi) to the P-site and binding of the first NTP substrate (NTPi+1) to the N-site.	bind
49984	7	10921	5	13	NULL	NULL	NULL	statement 5	Process		involves					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24991_s_173	16831816	A minimum requirement for  de novo initiation of RNA synthesis by BVDV and HCV RdRps involves binding of the initiating nucleotide (NTPi) to the P-site and binding of the first NTP substrate (NTPi+1) to the N-site.	bind
49985	8	10921	5	13	NULL	NULL	NULL	statement 5	Process		involves					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24991_s_173	16831816	A minimum requirement for  de novo initiation of RNA synthesis by BVDV and HCV RdRps involves binding of the initiating nucleotide (NTPi) to the P-site and binding of the first NTP substrate (NTPi+1) to the N-site.	bind
49986	9	10921	5	13	NULL	NULL	NULL	statement 6	Process		involves					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24991_s_173	16831816	A minimum requirement for  de novo initiation of RNA synthesis by BVDV and HCV RdRps involves binding of the initiating nucleotide (NTPi) to the P-site and binding of the first NTP substrate (NTPi+1) to the N-site.	bind
49987	10	10921	5	13	NULL	NULL	NULL	statement 6	Process		involves					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24991_s_173	16831816	A minimum requirement for  de novo initiation of RNA synthesis by BVDV and HCV RdRps involves binding of the initiating nucleotide (NTPi) to the P-site and binding of the first NTP substrate (NTPi+1) to the N-site.	bind
41960	1	10921	6	NULL	NULL	0	NULL	NTPi	NULL		is	NULL				initiating nucleotide	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_34_24991_s_173	16831816	A minimum requirement for  de novo initiation of RNA synthesis by BVDV and HCV RdRps involves binding of the initiating nucleotide (NTPi) to the P-site and binding of the first NTP substrate (NTPi+1) to the N-site.	bind
41962	2	10921	6	NULL	NULL	0	NULL	NTPi+1	NULL		is	NULL				first NTP substrate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_34_24991_s_173	16831816	A minimum requirement for  de novo initiation of RNA synthesis by BVDV and HCV RdRps involves binding of the initiating nucleotide (NTPi) to the P-site and binding of the first NTP substrate (NTPi+1) to the N-site.	bind
41963	3	10921	6	NULL	NULL	0	NULL	NTPi	NULL		bind	NULL					NULL		P-site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24991_s_173	16831816	A minimum requirement for  de novo initiation of RNA synthesis by BVDV and HCV RdRps involves binding of the initiating nucleotide (NTPi) to the P-site and binding of the first NTP substrate (NTPi+1) to the N-site.	bind
41964	4	10921	6	NULL	NULL	0	NULL	NTPi+1	NULL		bind	NULL					NULL		N-site		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_34_24991_s_173	16831816	A minimum requirement for  de novo initiation of RNA synthesis by BVDV and HCV RdRps involves binding of the initiating nucleotide (NTPi) to the P-site and binding of the first NTP substrate (NTPi+1) to the N-site.	bind
41966	5	10921	6	NULL	NULL	0	NULL	BVDV	NULL		initiates	NULL				RNA	NULL	de novo synthesis of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_34_24991_s_173	16831816	A minimum requirement for  de novo initiation of RNA synthesis by BVDV and HCV RdRps involves binding of the initiating nucleotide (NTPi) to the P-site and binding of the first NTP substrate (NTPi+1) to the N-site.	bind
41968	6	10921	6	NULL	NULL	0	NULL	HCV RdRps	NULL		initiates	NULL				RNA	NULL	de novo synthesis of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_34_24991_s_173	16831816	A minimum requirement for  de novo initiation of RNA synthesis by BVDV and HCV RdRps involves binding of the initiating nucleotide (NTPi) to the P-site and binding of the first NTP substrate (NTPi+1) to the N-site.	bind
41970	7	10921	6	NULL	NULL	0	NULL	statement 5	NULL		requires	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_34_24991_s_173	16831816	A minimum requirement for  de novo initiation of RNA synthesis by BVDV and HCV RdRps involves binding of the initiating nucleotide (NTPi) to the P-site and binding of the first NTP substrate (NTPi+1) to the N-site.	bind
41971	8	10921	6	NULL	NULL	0	NULL	statement 5	NULL		requires	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_34_24991_s_173	16831816	A minimum requirement for  de novo initiation of RNA synthesis by BVDV and HCV RdRps involves binding of the initiating nucleotide (NTPi) to the P-site and binding of the first NTP substrate (NTPi+1) to the N-site.	bind
41973	9	10921	6	NULL	NULL	0	NULL	statement 6	NULL		requires	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_34_24991_s_173	16831816	A minimum requirement for  de novo initiation of RNA synthesis by BVDV and HCV RdRps involves binding of the initiating nucleotide (NTPi) to the P-site and binding of the first NTP substrate (NTPi+1) to the N-site.	bind
41974	10	10921	6	NULL	NULL	0	NULL	statement 6	NULL		requires	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_34_24991_s_173	16831816	A minimum requirement for  de novo initiation of RNA synthesis by BVDV and HCV RdRps involves binding of the initiating nucleotide (NTPi) to the P-site and binding of the first NTP substrate (NTPi+1) to the N-site.	bind
49988	1	10922	5	13	NULL	NULL	NULL	Msbp-4	GP		is a type of					minisatellite-binding protein	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_267_17_1601895_s_2	1601895	A minisatellite-binding protein, Msbp-4, with a molecular mass of 35 kDa  has been purified from mouse tumor cells that binds to hypervariable Pc-1  and Pc-2 minisatellites.	bind
49989	2	10922	5	13	NULL	NULL	NULL	Pc-1	NucleicAcid		is a type of					hypervariable minisatellite	NucleicAcid				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_267_17_1601895_s_2	1601895	A minisatellite-binding protein, Msbp-4, with a molecular mass of 35 kDa  has been purified from mouse tumor cells that binds to hypervariable Pc-1  and Pc-2 minisatellites.	bind
49990	3	10922	5	13	NULL	NULL	NULL	Pc-2	NucleicAcid		is a type of					hypervariable minisatellite	NucleicAcid				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_267_17_1601895_s_2	1601895	A minisatellite-binding protein, Msbp-4, with a molecular mass of 35 kDa  has been purified from mouse tumor cells that binds to hypervariable Pc-1  and Pc-2 minisatellites.	bind
49991	4	10922	5	13	NULL	NULL	NULL	Msbp-4	GP		bind					Pc-1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_267_17_1601895_s_2	1601895	A minisatellite-binding protein, Msbp-4, with a molecular mass of 35 kDa  has been purified from mouse tumor cells that binds to hypervariable Pc-1  and Pc-2 minisatellites.	bind
49992	5	10922	5	13	NULL	NULL	NULL	Msbp-4	GP		bind					Pc-2	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_267_17_1601895_s_2	1601895	A minisatellite-binding protein, Msbp-4, with a molecular mass of 35 kDa  has been purified from mouse tumor cells that binds to hypervariable Pc-1  and Pc-2 minisatellites.	bind
41976	1	10922	6	NULL	NULL	0	NULL	Msbp-4	NULL		is a type of	NULL				minisatellite-binding protein	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_267_17_1601895_s_2	1601895	A minisatellite-binding protein, Msbp-4, with a molecular mass of 35 kDa  has been purified from mouse tumor cells that binds to hypervariable Pc-1  and Pc-2 minisatellites.	bind
41977	2	10922	6	NULL	NULL	0	NULL	Msbp-4	NULL		bind	NULL				Pc-1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_267_17_1601895_s_2	1601895	A minisatellite-binding protein, Msbp-4, with a molecular mass of 35 kDa  has been purified from mouse tumor cells that binds to hypervariable Pc-1  and Pc-2 minisatellites.	bind
41978	3	10922	6	NULL	NULL	0	NULL	Msbp-4	NULL		bind	NULL				Pc-2	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_267_17_1601895_s_2	1601895	A minisatellite-binding protein, Msbp-4, with a molecular mass of 35 kDa  has been purified from mouse tumor cells that binds to hypervariable Pc-1  and Pc-2 minisatellites.	bind
41979	4	10922	6	NULL	NULL	0	NULL	Pc-1	NULL		is a type of	NULL				hypervariable minisatellite	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_267_17_1601895_s_2	1601895	A minisatellite-binding protein, Msbp-4, with a molecular mass of 35 kDa  has been purified from mouse tumor cells that binds to hypervariable Pc-1  and Pc-2 minisatellites.	bind
41980	5	10922	6	NULL	NULL	0	NULL	Pc-2	NULL		is a type of	NULL				hypervariable minisatellite	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_267_17_1601895_s_2	1601895	A minisatellite-binding protein, Msbp-4, with a molecular mass of 35 kDa  has been purified from mouse tumor cells that binds to hypervariable Pc-1  and Pc-2 minisatellites.	bind
49993	1	10923	5	13	NULL	NULL	NULL	GST-GluR2	GP		bind					SAP97	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_31_19518_s_244	9677374	A minor amount of GST-GluR2 bound to SAP97 (Fig.  5,  lane 2), but GST-GluR2 binding was hardly detectable.	bind
41995	1	10923	6	NULL	NULL	0	NULL	GST-GluR2	NULL		bind	NULL				SAP97	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_31_19518_s_244	9677374	A minor amount of GST-GluR2 bound to SAP97 (Fig.  5,  lane 2), but GST-GluR2 binding was hardly detectable.	bind
49995	1	10925	5	13	NULL	NULL	NULL	PE2I	GP		bind					SERT	GP				NULL	cerebral area	NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_291_2_648_s_196	10525084	A minor binding of PE2I to the SERT can therefore not be excluded in this cerebral area.	bind
42007	1	10925	6	NULL	NULL	0	NULL	PE2I	NULL		bind	NULL				SERT	NULL				NULL	cerebral area	0	NULL	NULL	NULL	gw60_jpharmacolexpther_291_2_648_s_196	10525084	A minor binding of PE2I to the SERT can therefore not be excluded in this cerebral area.	bind
49996	1	10926	5	13	NULL	NULL	NULL	minor protein	GP		is present in					type 1 fimbriae	CellComponent	tip of			NULL		NULL	NULL	NULL	NULL	gw60_annurevmicrobiol_50_0_513_s_289	8905090	A minor protein at the tip of the type 1 fimbriae  possibly mediates the binding of  A. naeslundii T14V to  salivary proline-rich proteins ( 162).	bind
49997	2	10926	5	13	NULL	NULL	NULL			A. naeslundii	bind			T14V		proline-rich proteins	GP	salivary			NULL		NULL	NULL	NULL	NULL	gw60_annurevmicrobiol_50_0_513_s_289	8905090	A minor protein at the tip of the type 1 fimbriae  possibly mediates the binding of  A. naeslundii T14V to  salivary proline-rich proteins ( 162).	bind
49998	3	10926	5	13	NULL	NULL	NULL	statement 1	Process		mediate		possibly			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_annurevmicrobiol_50_0_513_s_289	8905090	A minor protein at the tip of the type 1 fimbriae  possibly mediates the binding of  A. naeslundii T14V to  salivary proline-rich proteins ( 162).	bind
42008	1	10926	6	NULL	NULL	0	NULL		NULL	A. naeslundii	bind	NULL		T14V		proline-rich proteins	NULL	salivary			NULL		0	NULL	NULL	NULL	gw60_annurevmicrobiol_50_0_513_s_289	8905090	A minor protein at the tip of the type 1 fimbriae  possibly mediates the binding of  A. naeslundii T14V to  salivary proline-rich proteins ( 162).	bind
42009	2	10926	6	10	NULL	0	NULL	minor protein	NULL		is present at	NULL				 type 1 fimbriae	NULL	tip of 			NULL		NULL	NULL	NULL	NULL	gw60_annurevmicrobiol_50_0_513_s_289	8905090	A minor protein at the tip of the type 1 fimbriae  possibly mediates the binding of  A. naeslundii T14V to  salivary proline-rich proteins ( 162).	bind
42010	3	10926	6	10	NULL	0	NULL	statement 2			mediates		possibly			statement 1					NULL		NULL	NULL	NULL	NULL	gw60_annurevmicrobiol_50_0_513_s_289	8905090	A minor protein at the tip of the type 1 fimbriae  possibly mediates the binding of  A. naeslundii T14V to  salivary proline-rich proteins ( 162).	bind
50013	1	10927	5	13	NULL	NULL	NULL	colicin E9	GP		is a type of					DNase	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_3_1286_s_174	11830660	A mismatch of the binding site on only one of the two helices, as occurs when colicin E9 DNase binds to the noncognate ImmE2, causes the binding constant to fall by six orders of magnitude ( 23).	bind
50014	2	10927	5	13	NULL	NULL	NULL	colicin E9	GP		bind					ImmE2	GP	noncognate			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_3_1286_s_174	11830660	A mismatch of the binding site on only one of the two helices, as occurs when colicin E9 DNase binds to the noncognate ImmE2, causes the binding constant to fall by six orders of magnitude ( 23).	bind
42011	1	10927	6	10	NULL	0	NULL	colicin E9	NULL		bind	NULL				ImmE2	NULL	noncognate 			NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_3_1286_s_174	11830660	A mismatch of the binding site on only one of the two helices, as occurs when colicin E9 DNase binds to the noncognate ImmE2, causes the binding constant to fall by six orders of magnitude ( 23).	bind
42012	2	10927	6	NULL	NULL	0	NULL	colicin E9	NULL		is a type of	NULL				DNase	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_3_1286_s_174	11830660	A mismatch of the binding site on only one of the two helices, as occurs when colicin E9 DNase binds to the noncognate ImmE2, causes the binding constant to fall by six orders of magnitude ( 23).	bind
50015	1	10929	5	13	NULL	NULL	NULL	Ena	GP		bind					zyxin	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molbiolcell_9_8_2157_s_7	9693373	A missense mutation that resulted in an amino acid substitution in the EVH1 domain eliminated in vitro binding of Ena to the cytoskeletal protein zyxin, a previously reported binding partner of VASP.	bind
50016	2	10929	5	13	NULL	NULL	NULL	zyxin	GP		is a type of					cytoskeletal protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_8_2157_s_7	9693373	A missense mutation that resulted in an amino acid substitution in the EVH1 domain eliminated in vitro binding of Ena to the cytoskeletal protein zyxin, a previously reported binding partner of VASP.	bind
50017	3	10929	5	13	NULL	NULL	NULL	zyxin	GP		bind					VASP	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_8_2157_s_7	9693373	A missense mutation that resulted in an amino acid substitution in the EVH1 domain eliminated in vitro binding of Ena to the cytoskeletal protein zyxin, a previously reported binding partner of VASP.	bind
50018	4	10929	5	13	NULL	NULL	NULL			missense mutation in	eliminates			EVH1 domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_8_2157_s_7	9693373	A missense mutation that resulted in an amino acid substitution in the EVH1 domain eliminated in vitro binding of Ena to the cytoskeletal protein zyxin, a previously reported binding partner of VASP.	bind
42013	1	10929	6	NULL	NULL	0	NULL	Ena	NULL		bind	NULL				zyxin	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_molbiolcell_9_8_2157_s_7	9693373	A missense mutation that resulted in an amino acid substitution in the EVH1 domain eliminated in vitro binding of Ena to the cytoskeletal protein zyxin, a previously reported binding partner of VASP.	bind
42014	2	10929	6	NULL	NULL	0	NULL	zyxin	NULL		is a type of	NULL				cytoskeletal protein	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_9_8_2157_s_7	9693373	A missense mutation that resulted in an amino acid substitution in the EVH1 domain eliminated in vitro binding of Ena to the cytoskeletal protein zyxin, a previously reported binding partner of VASP.	bind
42015	3	10929	6	NULL	NULL	0	NULL	zyxin	NULL		bind	NULL				VASP	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_9_8_2157_s_7	9693373	A missense mutation that resulted in an amino acid substitution in the EVH1 domain eliminated in vitro binding of Ena to the cytoskeletal protein zyxin, a previously reported binding partner of VASP.	bind
42016	4	10929	6	NULL	NULL	0	NULL		NULL	mutant	eliminates	NULL		EVH1 domain		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_9_8_2157_s_7	9693373	A missense mutation that resulted in an amino acid substitution in the EVH1 domain eliminated in vitro binding of Ena to the cytoskeletal protein zyxin, a previously reported binding partner of VASP.	bind
50019	1	10930	5	13	NULL	NULL	NULL	RBP16	GP		is a type of					mitochondrial Y-box protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_20_7010_s_331	11564883	A mitochondrial Y-box protein in  Trypanosoma brucei, RBP16, which binds guide RNAs (gRNAs) specifically in vitro, has been shown to interact with gRNAs in vivo ( 28).	bind
50020	2	10930	5	13	NULL	NULL	NULL	RBP16	GP	Trypanosoma brucei	bind		specifically			gRNAs	NucleicAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_20_7010_s_331	11564883	A mitochondrial Y-box protein in  Trypanosoma brucei, RBP16, which binds guide RNAs (gRNAs) specifically in vitro, has been shown to interact with gRNAs in vivo ( 28).	bind
50021	3	10930	5	13	NULL	NULL	NULL	RBP16	GP	Trypanosoma brucei	interacts with					gRNAs	NucleicAcid				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_20_7010_s_331	11564883	A mitochondrial Y-box protein in  Trypanosoma brucei, RBP16, which binds guide RNAs (gRNAs) specifically in vitro, has been shown to interact with gRNAs in vivo ( 28).	bind
50022	4	10930	5	13	NULL	NULL	NULL	gRNAs	NucleicAcid		is					guide RNAs	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_20_7010_s_331	11564883	A mitochondrial Y-box protein in  Trypanosoma brucei, RBP16, which binds guide RNAs (gRNAs) specifically in vitro, has been shown to interact with gRNAs in vivo ( 28).	bind
42017	1	10930	6	NULL	NULL	0	NULL	RBP16	NULL		is a type of	NULL				mitochondrial Y-box protein	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_20_7010_s_331	11564883	A mitochondrial Y-box protein in  Trypanosoma brucei, RBP16, which binds guide RNAs (gRNAs) specifically in vitro, has been shown to interact with gRNAs in vivo ( 28).	bind
42018	2	10930	6	NULL	NULL	0	NULL	gRNA	NULL		is	NULL				guide RNA	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_20_7010_s_331	11564883	A mitochondrial Y-box protein in  Trypanosoma brucei, RBP16, which binds guide RNAs (gRNAs) specifically in vitro, has been shown to interact with gRNAs in vivo ( 28).	bind
42019	3	10930	6	NULL	NULL	0	NULL	RBP16	NULL	Trypanosoma brucei	bind	NULL	specifically			gRNA	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_20_7010_s_331	11564883	A mitochondrial Y-box protein in  Trypanosoma brucei, RBP16, which binds guide RNAs (gRNAs) specifically in vitro, has been shown to interact with gRNAs in vivo ( 28).	bind
42020	4	10930	6	NULL	NULL	0	NULL	RBP16	NULL	Trypanosoma brucei	bind	NULL	specifically			gRNA	NULL				NULL	in vivo	0	NULL	NULL	NULL	gw60_molcellbiol_21_20_7010_s_331	11564883	A mitochondrial Y-box protein in  Trypanosoma brucei, RBP16, which binds guide RNAs (gRNAs) specifically in vitro, has been shown to interact with gRNAs in vivo ( 28).	bind
50023	1	10931	5	13	NULL	NULL	NULL	mitogen	Chemical		activates					Protein Kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6983_s_699	9819386	A Mitogen-activated Protein Kinase-dependent Signaling Pathway in the Activation of Platelet Integrin alpha IIbbeta 3.	bind
50024	2	10931	5	13	NULL	NULL	NULL	signaling pathway	Process		depends on					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6983_s_699	9819386	A Mitogen-activated Protein Kinase-dependent Signaling Pathway in the Activation of Platelet Integrin alpha IIbbeta 3.	bind
50025	3	10931	5	13	NULL	NULL	NULL	statement 2	Process		activates					Integrin alpha IIbbeta 3	GP	platelet			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6983_s_699	9819386	A Mitogen-activated Protein Kinase-dependent Signaling Pathway in the Activation of Platelet Integrin alpha IIbbeta 3.	bind
42021	1	10931	6	10	NULL	0	NULL	Mitogen	NULL		activates	NULL				Protein Kinase	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6983_s_699	9819386	A Mitogen-activated Protein Kinase-dependent Signaling Pathway in the Activation of Platelet Integrin alpha IIbbeta 3.	bind
42022	2	10931	6	10	NULL	0	NULL	signaling pathway	NULL		depends on	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6983_s_699	9819386	A Mitogen-activated Protein Kinase-dependent Signaling Pathway in the Activation of Platelet Integrin alpha IIbbeta 3.	bind
50480	3	10931	6	10	NULL	0	NULL	statement 2	NULL		activates	NULL				Integrin alpha IIbbeta 3	NULL	platelet			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_12_6983_s_699	9819386	A Mitogen-activated Protein Kinase-dependent Signaling Pathway in the Activation of Platelet Integrin alpha IIbbeta 3.	bind
50026	1	10932	5	13	NULL	NULL	NULL	mitotic kinesin-related protein	GP		bind					PP1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_10_5600_s_266	7890679	A Mitotic Kinesin-related Protein That Binds PP1.	bind
42023	1	10932	6	10	NULL	0	NULL	Mitotic Kinesin-related Protein	NULL		bind	NULL				PP1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_10_5600_s_266	7890679	A Mitotic Kinesin-related Protein That Binds PP1.	bind
50027	1	10933	5	13	NULL	NULL	NULL	aminopeptidase	GP	Manduca sexta	mixed with					alkaline phosphatase	GP				NULL		NULL	NULL	NULL	NULL	gw60_insectbiochemmolbiol_32_1_97_s_513	11719073	A mixture of  Manduca sexta aminopeptidase and alkaline phosphatase enhances  Bacillus thuringiensis insecticidal Cry1A(c) toxin binding and 86Rb+-K+ leakage in vitro.	bind
50028	2	10933	5	13	NULL	NULL	NULL	statement 1	Process		enhances					Cry1A(c)	Chemical	Bacillus thuringiensis;;binding of			NULL		NULL	NULL	NULL	NULL	gw60_insectbiochemmolbiol_32_1_97_s_513	11719073	A mixture of  Manduca sexta aminopeptidase and alkaline phosphatase enhances  Bacillus thuringiensis insecticidal Cry1A(c) toxin binding and 86Rb+-K+ leakage in vitro.	bind
50029	3	10933	5	13	NULL	NULL	NULL	Cry1A(c)	Chemical		is a type of					insecticidal toxin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_insectbiochemmolbiol_32_1_97_s_513	11719073	A mixture of  Manduca sexta aminopeptidase and alkaline phosphatase enhances  Bacillus thuringiensis insecticidal Cry1A(c) toxin binding and 86Rb+-K+ leakage in vitro.	bind
50030	4	10933	5	13	NULL	NULL	NULL	statement 1	Process		enhances					Rb+-K+	Chemical	leakage of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_insectbiochemmolbiol_32_1_97_s_513	11719073	A mixture of  Manduca sexta aminopeptidase and alkaline phosphatase enhances  Bacillus thuringiensis insecticidal Cry1A(c) toxin binding and 86Rb+-K+ leakage in vitro.	bind
42024	1	10933	6	NULL	NULL	0	NULL	aminopeptidase	NULL	Manduca sexta	forms a mixture with	NULL				alkaline phosphatase	NULL				NULL		0	NULL	NULL	NULL	gw60_insectbiochemmolbiol_32_1_97_s_513	11719073	A mixture of  Manduca sexta aminopeptidase and alkaline phosphatase enhances  Bacillus thuringiensis insecticidal Cry1A(c) toxin binding and 86Rb+-K+ leakage in vitro.	bind
42025	2	10933	6	NULL	NULL	0	NULL	statement 1	NULL		enhances	NULL				Rb+-K+	NULL	leakage of			NULL	in vitro	0	NULL	NULL	NULL	gw60_insectbiochemmolbiol_32_1_97_s_513	11719073	A mixture of  Manduca sexta aminopeptidase and alkaline phosphatase enhances  Bacillus thuringiensis insecticidal Cry1A(c) toxin binding and 86Rb+-K+ leakage in vitro.	bind
42026	3	10933	6	NULL	NULL	0	NULL	statement 1	NULL		enhances	NULL				Cry1A(c)	NULL	Bacillus thuringiensis;; binding of 			NULL		0	NULL	NULL	NULL	gw60_insectbiochemmolbiol_32_1_97_s_513	11719073	A mixture of  Manduca sexta aminopeptidase and alkaline phosphatase enhances  Bacillus thuringiensis insecticidal Cry1A(c) toxin binding and 86Rb+-K+ leakage in vitro.	bind
42027	4	10933	6	NULL	NULL	0	NULL	Cry1A(c)	NULL		is a type of	NULL				insecticidal toxin	NULL				NULL		0	NULL	NULL	NULL	gw60_insectbiochemmolbiol_32_1_97_s_513	11719073	A mixture of  Manduca sexta aminopeptidase and alkaline phosphatase enhances  Bacillus thuringiensis insecticidal Cry1A(c) toxin binding and 86Rb+-K+ leakage in vitro.	bind
50031	1	10934	5	13	NULL	NULL	NULL	aminopeptidase	GP	Manduca sexta	mixed with					phosphatase	GP				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_64_8_2995_s_526	9687463	A mixture of  Manduca sexta aminopeptidase and phosphatase enhances  Bacillus thuringiensis insecticidal Cry1A(c) toxin binding and 86Rb + efflux  in vitro.	bind
50032	2	10934	5	13	NULL	NULL	NULL	statement 1	Process		enhances					Cry1A(c)	Chemical	Bacillus thuringiensis;;binding of			NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_64_8_2995_s_526	9687463	A mixture of  Manduca sexta aminopeptidase and phosphatase enhances  Bacillus thuringiensis insecticidal Cry1A(c) toxin binding and 86Rb + efflux  in vitro.	bind
50033	3	10934	5	13	NULL	NULL	NULL	Cry1A(c)	Chemical		is a type of					insecticidal toxin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_64_8_2995_s_526	9687463	A mixture of  Manduca sexta aminopeptidase and phosphatase enhances  Bacillus thuringiensis insecticidal Cry1A(c) toxin binding and 86Rb + efflux  in vitro.	bind
50034	4	10934	5	13	NULL	NULL	NULL	statement 1	Process		enhances					Rb + efflux	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_applenvironmicrob_64_8_2995_s_526	9687463	A mixture of  Manduca sexta aminopeptidase and phosphatase enhances  Bacillus thuringiensis insecticidal Cry1A(c) toxin binding and 86Rb + efflux  in vitro.	bind
50035	1	10937	5	13	NULL	NULL	NULL	GST-EBP50	GP		bind					ezrin	GP		N-ERMAD		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7621_s_233	11106646	A mixture of the two N-ERMADs used is shown in  lane L. B, competitive binding of GST-EBP50 ( EBP) and ezrin C-ERMAD ( EzC) or merlin C-ERMAD ( MrC) to ezrin N-ERMAD beads.	bind
50036	2	10937	5	13	NULL	NULL	NULL	ezrin	GP		bind			C-ERMAD		ezrin	GP		N-ERMAD		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7621_s_233	11106646	A mixture of the two N-ERMADs used is shown in  lane L. B, competitive binding of GST-EBP50 ( EBP) and ezrin C-ERMAD ( EzC) or merlin C-ERMAD ( MrC) to ezrin N-ERMAD beads.	bind
50037	3	10937	5	13	NULL	NULL	NULL	merlin	GP		bind			C-ERMAD		ezrin	GP		N-ERMAD		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7621_s_233	11106646	A mixture of the two N-ERMADs used is shown in  lane L. B, competitive binding of GST-EBP50 ( EBP) and ezrin C-ERMAD ( EzC) or merlin C-ERMAD ( MrC) to ezrin N-ERMAD beads.	bind
50038	4	10937	5	13	NULL	NULL	NULL	statement 1	Process		competes with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7621_s_233	11106646	A mixture of the two N-ERMADs used is shown in  lane L. B, competitive binding of GST-EBP50 ( EBP) and ezrin C-ERMAD ( EzC) or merlin C-ERMAD ( MrC) to ezrin N-ERMAD beads.	bind
50039	5	10937	5	13	NULL	NULL	NULL	statement 1	Process		competes with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7621_s_233	11106646	A mixture of the two N-ERMADs used is shown in  lane L. B, competitive binding of GST-EBP50 ( EBP) and ezrin C-ERMAD ( EzC) or merlin C-ERMAD ( MrC) to ezrin N-ERMAD beads.	bind
42068	1	10937	6	NULL	NULL	0	NULL	GST-EBP50	NULL		bind	NULL				ezrin	NULL		N-ERMAD		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_10_7621_s_233	11106646	A mixture of the two N-ERMADs used is shown in  lane L. B, competitive binding of GST-EBP50 ( EBP) and ezrin C-ERMAD ( EzC) or merlin C-ERMAD ( MrC) to ezrin N-ERMAD beads.	bind
42069	2	10937	6	NULL	NULL	0	NULL	ezrin	NULL		bind	NULL		C-ERMAD		ezrin	NULL		N-ERMAD		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_10_7621_s_233	11106646	A mixture of the two N-ERMADs used is shown in  lane L. B, competitive binding of GST-EBP50 ( EBP) and ezrin C-ERMAD ( EzC) or merlin C-ERMAD ( MrC) to ezrin N-ERMAD beads.	bind
42070	3	10937	6	NULL	NULL	0	NULL	statement 1	NULL		competes	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_10_7621_s_233	11106646	A mixture of the two N-ERMADs used is shown in  lane L. B, competitive binding of GST-EBP50 ( EBP) and ezrin C-ERMAD ( EzC) or merlin C-ERMAD ( MrC) to ezrin N-ERMAD beads.	bind
42071	4	10937	6	NULL	NULL	0	NULL	merlin	NULL		bind	NULL		C-ERMAD		ezrin	NULL		N-ERMAD		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_10_7621_s_233	11106646	A mixture of the two N-ERMADs used is shown in  lane L. B, competitive binding of GST-EBP50 ( EBP) and ezrin C-ERMAD ( EzC) or merlin C-ERMAD ( MrC) to ezrin N-ERMAD beads.	bind
42072	5	10937	6	NULL	NULL	0	NULL	statement 1	NULL		competes	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_10_7621_s_233	11106646	A mixture of the two N-ERMADs used is shown in  lane L. B, competitive binding of GST-EBP50 ( EBP) and ezrin C-ERMAD ( EzC) or merlin C-ERMAD ( MrC) to ezrin N-ERMAD beads.	bind
50040	1	10939	5	13	NULL	NULL	NULL	Gal4p	GP		bind					episomal DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_11_7612_s_183	10713069	A MN cleavage site with very similar characteristic has been recently described in the case of Gal4p binding to episomal DNA ( 43).	bind
42028	1	10939	6	NULL	NULL	0	NULL	Gal4p	NULL		bind	NULL				episomal DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_11_7612_s_183	10713069	A MN cleavage site with very similar characteristic has been recently described in the case of Gal4p binding to episomal DNA ( 43).	bind
50041	1	10941	5	13	NULL	NULL	NULL	TLF	GP		mediates					trypanosomes	Organism	lysis of			NULL		NULL	NULL	NULL	NULL	gw70_clinmicrobiolrev_12_1_112_s_162	9880477	A model ( ) has been proposed which recognizes three phases in the process of TLF-mediated lysis of trypanosomes: (i) binding of TLF to a trypanosome receptor, (ii) internalization by endocytosis, and (iii) lysosomal targeting.	bind
50042	2	10941	5	13	NULL	NULL	NULL	TLF	GP		bind					trypanosome receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_clinmicrobiolrev_12_1_112_s_162	9880477	A model ( ) has been proposed which recognizes three phases in the process of TLF-mediated lysis of trypanosomes: (i) binding of TLF to a trypanosome receptor, (ii) internalization by endocytosis, and (iii) lysosomal targeting.	bind
42029	1	10941	6	NULL	NULL	0	NULL	TLF	NULL		bind	NULL				trypanosome receptor	NULL				NULL		0	NULL	NULL	NULL	gw70_clinmicrobiolrev_12_1_112_s_162	9880477	A model ( ) has been proposed which recognizes three phases in the process of TLF-mediated lysis of trypanosomes: (i) binding of TLF to a trypanosome receptor, (ii) internalization by endocytosis, and (iii) lysosomal targeting.	bind
50481	2	10941	6	10	NULL	0	NULL	TLF	NULL		mediates	NULL				trypanosomes	NULL	lysis of			NULL		0	NULL	NULL	NULL	gw70_clinmicrobiolrev_12_1_112_s_162	9880477	A model ( ) has been proposed which recognizes three phases in the process of TLF-mediated lysis of trypanosomes: (i) binding of TLF to a trypanosome receptor, (ii) internalization by endocytosis, and (iii) lysosomal targeting.	bind
50043	1	10943	5	13	NULL	NULL	NULL	PICK1	GP		bind					GluR2	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_52_18212_s_17	15608060	A model based on these findings proposes that PICK1 binds GluR2 after protein kinase C-mediated phosphorylation at Ser-880.	bind
50044	2	10943	5	13	NULL	NULL	NULL	protein kinase C	GP		mediates							phosphorylation	Ser-880		NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_52_18212_s_17	15608060	A model based on these findings proposes that PICK1 binds GluR2 after protein kinase C-mediated phosphorylation at Ser-880.	bind
50045	3	10943	5	13	NULL	NULL	NULL	statement 1	Process		occurs after					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_52_18212_s_17	15608060	A model based on these findings proposes that PICK1 binds GluR2 after protein kinase C-mediated phosphorylation at Ser-880.	bind
42030	1	10943	6	NULL	NULL	0	NULL	PICK1	NULL		bind	NULL				GluR2	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_101_52_18212_s_17	15608060	A model based on these findings proposes that PICK1 binds GluR2 after protein kinase C-mediated phosphorylation at Ser-880.	bind
42031	2	10943	6	NULL	NULL	0	NULL	protein kinase C	NULL		mediates	NULL					NULL	phosphorylation at	Ser-880		NULL		0	NULL	NULL	NULL	gw70_pnas_101_52_18212_s_17	15608060	A model based on these findings proposes that PICK1 binds GluR2 after protein kinase C-mediated phosphorylation at Ser-880.	bind
42032	3	10943	6	NULL	NULL	0	NULL	statement 1	NULL		occurs after	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_101_52_18212_s_17	15608060	A model based on these findings proposes that PICK1 binds GluR2 after protein kinase C-mediated phosphorylation at Ser-880.	bind
50046	1	10944	5	13	NULL	NULL	NULL	adducin tails	GP		bind					actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_14_7986_s_134	8626479	A model depicting binding  of adducin tails to actin and capping the barbed end of the actin  filament by adducin heads is shown in  Fig. 5 .	bind
50047	2	10944	5	13	NULL	NULL	NULL	adducin heads	GP		caps					actin filament	GP	barbed end of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_14_7986_s_134	8626479	A model depicting binding  of adducin tails to actin and capping the barbed end of the actin  filament by adducin heads is shown in  Fig. 5 .	bind
42033	1	10944	6	NULL	NULL	0	NULL	adducin tails	NULL		bind	NULL				actin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_7986_s_134	8626479	A model depicting binding  of adducin tails to actin and capping the barbed end of the actin  filament by adducin heads is shown in  Fig. 5 .	bind
50482	2	10944	6	10	NULL	0	NULL	adducin heads	NULL		caps	NULL				actin filaments	NULL	barbed end of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_7986_s_134	8626479	A model depicting binding  of adducin tails to actin and capping the barbed end of the actin  filament by adducin heads is shown in  Fig. 5 .	bind
50048	1	10945	5	13	NULL	NULL	NULL	PP2A	GP		interacts with					CK2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_49_34669_s_217	10574932	A model depicting regulation of Sp1 binding by  PP2A  interacting with  CK2  at basal and MAPK-signaled activation of  eNOS  gene transcription.	bind
50049	2	10945	5	13	NULL	NULL	NULL	statement 1	Process		regulates					Sp1	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_49_34669_s_217	10574932	A model depicting regulation of Sp1 binding by  PP2A  interacting with  CK2  at basal and MAPK-signaled activation of  eNOS  gene transcription.	bind
50050	3	10945	5	13	NULL	NULL	NULL	eNOS gene	GP	activation of ;;transcription of	is signaled by					MAPK	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_49_34669_s_217	10574932	A model depicting regulation of Sp1 binding by  PP2A  interacting with  CK2  at basal and MAPK-signaled activation of  eNOS  gene transcription.	bind
42073	1	10945	6	NULL	NULL	0	NULL	PP2A	NULL		interacts with	NULL				CK2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_49_34669_s_217	10574932	A model depicting regulation of Sp1 binding by  PP2A  interacting with  CK2  at basal and MAPK-signaled activation of  eNOS  gene transcription.	bind
42074	2	10945	6	10	NULL	0	NULL	MAPK	NULL		signals	NULL				eNOS gene 	NULL	activation of;;transcription of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_49_34669_s_217	10574932	A model depicting regulation of Sp1 binding by  PP2A  interacting with  CK2  at basal and MAPK-signaled activation of  eNOS  gene transcription.	bind
42075	3	10945	6	NULL	NULL	0	NULL	statement 1	NULL		regulates	NULL				Sp1	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_49_34669_s_217	10574932	A model depicting regulation of Sp1 binding by  PP2A  interacting with  CK2  at basal and MAPK-signaled activation of  eNOS  gene transcription.	bind
50052	1	10946	5	13	NULL	NULL	NULL	Argos	GP		is a type of					epidermal growth factor-like negative regulator 	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_42_27734_s_213	9765311	A model depicting the way agonists and antagonists may cooperate to control function is offered by  Drosophila, in which the epidermal growth factor-like negative regulator Argos binds to the mammalian epidermal growth factor receptor homologue ( Drosophila EGF receptor or DER), thereby preventing its activation by Spitz.	bind
50053	2	10946	5	13	NULL	NULL	NULL	Argos	GP	Drosophila	bind					DER	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_42_27734_s_213	9765311	A model depicting the way agonists and antagonists may cooperate to control function is offered by  Drosophila, in which the epidermal growth factor-like negative regulator Argos binds to the mammalian epidermal growth factor receptor homologue ( Drosophila EGF receptor or DER), thereby preventing its activation by Spitz.	bind
50054	3	10946	5	13	NULL	NULL	NULL	DER	GP		is					Drosophila EGF receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_42_27734_s_213	9765311	A model depicting the way agonists and antagonists may cooperate to control function is offered by  Drosophila, in which the epidermal growth factor-like negative regulator Argos binds to the mammalian epidermal growth factor receptor homologue ( Drosophila EGF receptor or DER), thereby preventing its activation by Spitz.	bind
50055	4	10946	5	13	NULL	NULL	NULL	DER	GP		is a homolog of					mammalian epidermal growth factor receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_42_27734_s_213	9765311	A model depicting the way agonists and antagonists may cooperate to control function is offered by  Drosophila, in which the epidermal growth factor-like negative regulator Argos binds to the mammalian epidermal growth factor receptor homologue ( Drosophila EGF receptor or DER), thereby preventing its activation by Spitz.	bind
50056	5	10946	5	13	NULL	NULL	NULL	Spitz	GP		activates					DER	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_42_27734_s_213	9765311	A model depicting the way agonists and antagonists may cooperate to control function is offered by  Drosophila, in which the epidermal growth factor-like negative regulator Argos binds to the mammalian epidermal growth factor receptor homologue ( Drosophila EGF receptor or DER), thereby preventing its activation by Spitz.	bind
50057	6	10946	5	13	NULL	NULL	NULL	statement 2	Process		prevents					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_42_27734_s_213	9765311	A model depicting the way agonists and antagonists may cooperate to control function is offered by  Drosophila, in which the epidermal growth factor-like negative regulator Argos binds to the mammalian epidermal growth factor receptor homologue ( Drosophila EGF receptor or DER), thereby preventing its activation by Spitz.	bind
42076	1	10946	6	NULL	NULL	0	NULL	Argos	NULL		is a type of	NULL				epidermal growth factor-like negative regulator	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_42_27734_s_213	9765311	A model depicting the way agonists and antagonists may cooperate to control function is offered by  Drosophila, in which the epidermal growth factor-like negative regulator Argos binds to the mammalian epidermal growth factor receptor homologue ( Drosophila EGF receptor or DER), thereby preventing its activation by Spitz.	bind
42077	2	10946	6	NULL	NULL	0	NULL	Argos	NULL	Drosophila	bind	NULL				DER	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_42_27734_s_213	9765311	A model depicting the way agonists and antagonists may cooperate to control function is offered by  Drosophila, in which the epidermal growth factor-like negative regulator Argos binds to the mammalian epidermal growth factor receptor homologue ( Drosophila EGF receptor or DER), thereby preventing its activation by Spitz.	bind
42078	3	10946	6	NULL	NULL	0	NULL	DER	NULL		is	NULL				Drosophila EGF receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_42_27734_s_213	9765311	A model depicting the way agonists and antagonists may cooperate to control function is offered by  Drosophila, in which the epidermal growth factor-like negative regulator Argos binds to the mammalian epidermal growth factor receptor homologue ( Drosophila EGF receptor or DER), thereby preventing its activation by Spitz.	bind
42079	4	10946	6	10	NULL	0	NULL	DER	NULL		is a homolog of	NULL				mammalian epidermal growth factor receptor	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_42_27734_s_213	9765311	A model depicting the way agonists and antagonists may cooperate to control function is offered by  Drosophila, in which the epidermal growth factor-like negative regulator Argos binds to the mammalian epidermal growth factor receptor homologue ( Drosophila EGF receptor or DER), thereby preventing its activation by Spitz.	bind
42080	5	10946	6	NULL	NULL	0	NULL	Spitz	NULL		activates	NULL				DER	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_42_27734_s_213	9765311	A model depicting the way agonists and antagonists may cooperate to control function is offered by  Drosophila, in which the epidermal growth factor-like negative regulator Argos binds to the mammalian epidermal growth factor receptor homologue ( Drosophila EGF receptor or DER), thereby preventing its activation by Spitz.	bind
42081	6	10946	6	NULL	NULL	0	NULL	statement 2	NULL		prevents	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_42_27734_s_213	9765311	A model depicting the way agonists and antagonists may cooperate to control function is offered by  Drosophila, in which the epidermal growth factor-like negative regulator Argos binds to the mammalian epidermal growth factor receptor homologue ( Drosophila EGF receptor or DER), thereby preventing its activation by Spitz.	bind
50058	1	10947	5	13	NULL	NULL	NULL	TPL-2	GP		bind					LPS	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_biochem-j_393_pt-3_16229681_s_12	16229681	A model describing  TPL-2 binding with LPS is proposed.	bind
42034	1	10947	6	NULL	NULL	0	NULL	TPL-2	NULL		bind	NULL				LPS	NULL				NULL		0	NULL	NULL	NULL	abs-batch0570-0579_biochem-j_393_pt-3_16229681_s_12	16229681	A model describing  TPL-2 binding with LPS is proposed.	bind
50059	1	10948	5	13	NULL	NULL	NULL	transcription factor	GP		bind									Region A sequence	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_8_6153_s_218	11748224	A model describing transcription factor binding to the Region A sequence, and the effects of mutations in the CCAAT-box and addition of mithramycin ( M) on binding, is illustrated in Fig.  5 B where  R represents the putative repressor binding to the GC-box.	bind
50061	2	10948	5	13	NULL	NULL	NULL	repressor	GP	putative	bind									GC-box	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_8_6153_s_218	11748224	A model describing transcription factor binding to the Region A sequence, and the effects of mutations in the CCAAT-box and addition of mithramycin ( M) on binding, is illustrated in Fig.  5 B where  R represents the putative repressor binding to the GC-box.	bind
42035	1	10948	6	NULL	NULL	0	NULL	repressor	NULL	putative	bind	NULL					NULL			GC-box	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_8_6153_s_218	11748224	A model describing transcription factor binding to the Region A sequence, and the effects of mutations in the CCAAT-box and addition of mithramycin ( M) on binding, is illustrated in Fig.  5 B where  R represents the putative repressor binding to the GC-box.	bind
42036	2	10948	6	NULL	NULL	0	NULL	transcription factor	NULL		bind	NULL					NULL			region A sequence	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_8_6153_s_218	11748224	A model describing transcription factor binding to the Region A sequence, and the effects of mutations in the CCAAT-box and addition of mithramycin ( M) on binding, is illustrated in Fig.  5 B where  R represents the putative repressor binding to the GC-box.	bind
50062	1	10949	5	13	NULL	NULL	NULL	tRNAPhe	NucleicAcid		bind					GAPDH	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1432_2_222_s_169	10407144	A model exhibiting the binding of tRNAPhe to GAPDH is shown in  Fig. 4.	bind
42037	1	10949	6	NULL	NULL	0	NULL	tRNAPhe	NULL		bind	NULL				GAPDH	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1432_2_222_s_169	10407144	A model exhibiting the binding of tRNAPhe to GAPDH is shown in  Fig. 4.	bind
50063	1	10950	5	13	NULL	NULL	NULL	L5	GP		bind			amino-terminal domain		5 S rRNA	NucleicAcid				NULL	nucleoplasm	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_19_11571_s_108	8626719	A model for 5 S rRNA trafficking can be formulated  where the L5 amino-terminal domain binds to 5 S rRNA shortly after  transcription in the nucleoplasm and the RNP then localizes to the  nucleolus by virtue of interactions between a nucleolar component and  the carboxyl-terminal domain of L5.	bind
50064	2	10950	5	13	NULL	NULL	NULL	statement 1	Process		occurs after		shortly			transcription	Process				NULL	nucleoplasm	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_19_11571_s_108	8626719	A model for 5 S rRNA trafficking can be formulated  where the L5 amino-terminal domain binds to 5 S rRNA shortly after  transcription in the nucleoplasm and the RNP then localizes to the  nucleolus by virtue of interactions between a nucleolar component and  the carboxyl-terminal domain of L5.	bind
50065	3	10950	5	13	NULL	NULL	NULL	RNP	GP		localize to					nucleolus	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_19_11571_s_108	8626719	A model for 5 S rRNA trafficking can be formulated  where the L5 amino-terminal domain binds to 5 S rRNA shortly after  transcription in the nucleoplasm and the RNP then localizes to the  nucleolus by virtue of interactions between a nucleolar component and  the carboxyl-terminal domain of L5.	bind
50066	4	10950	5	13	NULL	NULL	NULL	statement 1	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_19_11571_s_108	8626719	A model for 5 S rRNA trafficking can be formulated  where the L5 amino-terminal domain binds to 5 S rRNA shortly after  transcription in the nucleoplasm and the RNP then localizes to the  nucleolus by virtue of interactions between a nucleolar component and  the carboxyl-terminal domain of L5.	bind
50067	5	10950	5	13	NULL	NULL	NULL	nucleolar component	CellComponent		interacts with					L5	GP		carboxyl-terminal domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_19_11571_s_108	8626719	A model for 5 S rRNA trafficking can be formulated  where the L5 amino-terminal domain binds to 5 S rRNA shortly after  transcription in the nucleoplasm and the RNP then localizes to the  nucleolus by virtue of interactions between a nucleolar component and  the carboxyl-terminal domain of L5.	bind
42038	1	10950	6	NULL	NULL	0	NULL	L5	NULL		bind	NULL		amino-terminal domain		5S rRNA	NULL				NULL	nucleoplasm	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_19_11571_s_108	8626719	A model for 5 S rRNA trafficking can be formulated  where the L5 amino-terminal domain binds to 5 S rRNA shortly after  transcription in the nucleoplasm and the RNP then localizes to the  nucleolus by virtue of interactions between a nucleolar component and  the carboxyl-terminal domain of L5.	bind
42082	2	10950	6	10	NULL	0	NULL	statement 1	NULL		occurs after	NULL				transcription	NULL				NULL	nucleoplasm	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_19_11571_s_108	8626719	A model for 5 S rRNA trafficking can be formulated  where the L5 amino-terminal domain binds to 5 S rRNA shortly after  transcription in the nucleoplasm and the RNP then localizes to the  nucleolus by virtue of interactions between a nucleolar component and  the carboxyl-terminal domain of L5.	bind
42083	3	10950	6	NULL	NULL	0	NULL	RNP	NULL		localizes to	NULL				nucleolus	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_19_11571_s_108	8626719	A model for 5 S rRNA trafficking can be formulated  where the L5 amino-terminal domain binds to 5 S rRNA shortly after  transcription in the nucleoplasm and the RNP then localizes to the  nucleolus by virtue of interactions between a nucleolar component and  the carboxyl-terminal domain of L5.	bind
42084	4	10950	6	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_19_11571_s_108	8626719	A model for 5 S rRNA trafficking can be formulated  where the L5 amino-terminal domain binds to 5 S rRNA shortly after  transcription in the nucleoplasm and the RNP then localizes to the  nucleolus by virtue of interactions between a nucleolar component and  the carboxyl-terminal domain of L5.	bind
42569	5	10950	6	NULL	NULL	0	NULL	L5	NULL		bind	NULL		carboxyl-terminal domain		RNP	NULL		nucleolar component		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_19_11571_s_108	8626719	A model for 5 S rRNA trafficking can be formulated  where the L5 amino-terminal domain binds to 5 S rRNA shortly after  transcription in the nucleoplasm and the RNP then localizes to the  nucleolus by virtue of interactions between a nucleolar component and  the carboxyl-terminal domain of L5.	bind
50068	1	10951	5	13	NULL	NULL	NULL	ANP	GP		bind								extracellular domain		NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_68_0_127_s_146	10872446	A model for activation of GC-A, then, is that ANP binding to the   extracellular domain and ATP binding to the kinase homology domain lead to a   conformational change relieving kinase homology domain inhibition of the   catalytic domain.	bind
50069	2	10951	5	13	NULL	NULL	NULL	ATP	Chemical		bind								kinase homology domain		NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_68_0_127_s_146	10872446	A model for activation of GC-A, then, is that ANP binding to the   extracellular domain and ATP binding to the kinase homology domain lead to a   conformational change relieving kinase homology domain inhibition of the   catalytic domain.	bind
50070	3	10951	5	13	NULL	NULL	NULL	statement 1	Process		leads to					conformational change	Process				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_68_0_127_s_146	10872446	A model for activation of GC-A, then, is that ANP binding to the   extracellular domain and ATP binding to the kinase homology domain lead to a   conformational change relieving kinase homology domain inhibition of the   catalytic domain.	bind
50071	4	10951	5	NULL	NULL	0	NULL		NULL		inhibits	NULL		kinase homology domain			NULL		catalytic domain		NULL		0	NULL	NULL	NULL	gw60_annrevbiochem_68_0_127_s_146	10872446	A model for activation of GC-A, then, is that ANP binding to the   extracellular domain and ATP binding to the kinase homology domain lead to a   conformational change relieving kinase homology domain inhibition of the   catalytic domain.	bind
50072	5	10951	5	13	NULL	NULL	NULL	statement 3	Process		relieves					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_68_0_127_s_146	10872446	A model for activation of GC-A, then, is that ANP binding to the   extracellular domain and ATP binding to the kinase homology domain lead to a   conformational change relieving kinase homology domain inhibition of the   catalytic domain.	bind
50073	6	10951	5	13	NULL	NULL	NULL	statement 2	Process		leads to					conformational change	Process				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_68_0_127_s_146	10872446	A model for activation of GC-A, then, is that ANP binding to the   extracellular domain and ATP binding to the kinase homology domain lead to a   conformational change relieving kinase homology domain inhibition of the   catalytic domain.	bind
50074	7	10951	5	13	NULL	NULL	NULL	statement 6	Process		relieves					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_68_0_127_s_146	10872446	A model for activation of GC-A, then, is that ANP binding to the   extracellular domain and ATP binding to the kinase homology domain lead to a   conformational change relieving kinase homology domain inhibition of the   catalytic domain.	bind
42039	1	10951	6	NULL	NULL	0	NULL	ANP	NULL		bind	NULL					NULL		extracellular domain		NULL		0	NULL	NULL	NULL	gw60_annrevbiochem_68_0_127_s_146	10872446	A model for activation of GC-A, then, is that ANP binding to the   extracellular domain and ATP binding to the kinase homology domain lead to a   conformational change relieving kinase homology domain inhibition of the   catalytic domain.	bind
42040	2	10951	6	NULL	NULL	0	NULL	ATP	NULL		bind	NULL					NULL		kinase homology domain		NULL		0	NULL	NULL	NULL	gw60_annrevbiochem_68_0_127_s_146	10872446	A model for activation of GC-A, then, is that ANP binding to the   extracellular domain and ATP binding to the kinase homology domain lead to a   conformational change relieving kinase homology domain inhibition of the   catalytic domain.	bind
42041	3	10951	6	NULL	NULL	0	NULL		NULL		inhibits	NULL		kinase homology domain			NULL		catalytic domain		NULL		0	NULL	NULL	NULL	gw60_annrevbiochem_68_0_127_s_146	10872446	A model for activation of GC-A, then, is that ANP binding to the   extracellular domain and ATP binding to the kinase homology domain lead to a   conformational change relieving kinase homology domain inhibition of the   catalytic domain.	bind
42042	4	10951	6	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				conformational change	NULL				NULL		0	NULL	NULL	NULL	gw60_annrevbiochem_68_0_127_s_146	10872446	A model for activation of GC-A, then, is that ANP binding to the   extracellular domain and ATP binding to the kinase homology domain lead to a   conformational change relieving kinase homology domain inhibition of the   catalytic domain.	bind
42043	5	10951	6	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				conformational change	NULL				NULL		0	NULL	NULL	NULL	gw60_annrevbiochem_68_0_127_s_146	10872446	A model for activation of GC-A, then, is that ANP binding to the   extracellular domain and ATP binding to the kinase homology domain lead to a   conformational change relieving kinase homology domain inhibition of the   catalytic domain.	bind
42044	6	10951	6	NULL	NULL	0	NULL	statement 4	NULL		relieves	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_annrevbiochem_68_0_127_s_146	10872446	A model for activation of GC-A, then, is that ANP binding to the   extracellular domain and ATP binding to the kinase homology domain lead to a   conformational change relieving kinase homology domain inhibition of the   catalytic domain.	bind
42045	7	10951	6	NULL	NULL	0	NULL	statement 5	NULL		relieves	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_annrevbiochem_68_0_127_s_146	10872446	A model for activation of GC-A, then, is that ANP binding to the   extracellular domain and ATP binding to the kinase homology domain lead to a   conformational change relieving kinase homology domain inhibition of the   catalytic domain.	bind
50075	1	10952	5	13	NULL	NULL	NULL	AGRP	GP		bind					MCRs	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_20_14100_s_146	10318826	A model for AGRP binding to the MCRs remains to be developed.	bind
42046	1	10952	6	NULL	NULL	0	NULL	AGRP	NULL		bind	NULL				MCR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_20_14100_s_146	10318826	A model for AGRP binding to the MCRs remains to be developed.	bind
50076	1	10953	5	13	NULL	NULL	NULL	DnaA monomers	GP		bind					oriC	NucleicAcid			DnaA box	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_48_44919_s_213	11551962	A Model for Assembly of the Prepriming Complex--  In this model (Fig.  6), DnaA monomers bound to each DnaA box in  oriC creates a structure recognized by the DnaB-DnaC complex.	bind
50077	2	10953	5	13	NULL	NULL	NULL	statement 1	GP		is recognized by					DnaB-DnaC complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_48_44919_s_213	11551962	A Model for Assembly of the Prepriming Complex--  In this model (Fig.  6), DnaA monomers bound to each DnaA box in  oriC creates a structure recognized by the DnaB-DnaC complex.	bind
42047	1	10953	6	NULL	NULL	0	NULL	DnaA monomers	NULL		bind	NULL				oriC	NULL			DnaA box	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_48_44919_s_213	11551962	A Model for Assembly of the Prepriming Complex--  In this model (Fig.  6), DnaA monomers bound to each DnaA box in  oriC creates a structure recognized by the DnaB-DnaC complex.	bind
42048	2	10953	6	NULL	NULL	0	NULL	statement 1	NULL		is recognized by	NULL				DnaB-DnaC complex	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_48_44919_s_213	11551962	A Model for Assembly of the Prepriming Complex--  In this model (Fig.  6), DnaA monomers bound to each DnaA box in  oriC creates a structure recognized by the DnaB-DnaC complex.	bind
50078	1	10954	5	13	NULL	NULL	NULL	EG	Chemical		bind					mOR-EG	GP				NULL		NULL	NULL	NULL	NULL	gw70_jneurosci_25_7_1806_s_196	15716417	A model for binding of EG to mOR-EG and the orientation of amino acids in the binding  site.	bind
42085	1	10954	6	NULL	NULL	0	NULL	EG	NULL		bind	NULL				mOR-EG	NULL				NULL		0	NULL	NULL	NULL	gw70_jneurosci_25_7_1806_s_196	15716417	A model for binding of EG to mOR-EG and the orientation of amino acids in the binding  site.	bind
50079	1	10955	5	13	NULL	NULL	NULL	nitrite	Chemical		bind					NIR	GP	A. xylosoxidans			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_46_27458_s_343	7499203	A model for binding of nitrite to NIR from  A.  xylosoxidans  based on EXAFS studies ( 27 ) is not consistent  with our results.	bind
42128	1	10955	6	NULL	NULL	0	NULL	nitrite	NULL		bind	NULL				NIR	NULL	A. xylosoxidans			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_46_27458_s_343	7499203	A model for binding of nitrite to NIR from  A.  xylosoxidans  based on EXAFS studies ( 27 ) is not consistent  with our results.	bind
50080	1	10956	5	13	NULL	NULL	NULL	G9I peptide	GP		bind					Dd	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_2_1151_s_304	14583622	A model for binding of peptides G9I and Q11I to Dd.	bind
50081	2	10956	5	13	NULL	NULL	NULL	Q11I peptide	GP		bind					Dd	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_2_1151_s_304	14583622	A model for binding of peptides G9I and Q11I to Dd.	bind
42129	1	10956	6	NULL	NULL	0	NULL	G9I peptide	NULL		bind	NULL				Dd	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_2_1151_s_304	14583622	A model for binding of peptides G9I and Q11I to Dd.	bind
42131	2	10956	6	NULL	NULL	0	NULL	Q11I peptide	NULL		bind	NULL				Dd	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_2_1151_s_304	14583622	A model for binding of peptides G9I and Q11I to Dd.	bind
50082	1	10957	5	13	NULL	NULL	NULL	S1P	GP		bind					S1P1	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_270_s_225	12069838	A model for binding of S1P to S1P1 indicates that the polar head group of the ligand is situated in a polar region of the receptor near the extracellular surface, while the fatty acid tail is inserted into the receptor within its transmembrane domains [  67].	bind
42195	1	10957	6	NULL	NULL	0	NULL	S1P	NULL		bind	NULL		polar head group;; fatty acid tail		S1P1	NULL		polar region;; transmembrane domain		NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_270_s_225	12069838	A model for binding of S1P to S1P1 indicates that the polar head group of the ligand is situated in a polar region of the receptor near the extracellular surface, while the fatty acid tail is inserted into the receptor within its transmembrane domains [  67].	bind
50083	1	10959	5	13	NULL	NULL	NULL	thermolysin	GP		is a type of					metallopeptidase	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_41_39497_s_169	12888578	A model for catalysis based on the metallopeptidase thermolysin proposes that the internal glutamic acid polarizes the zinc-bound water molecule for a nucleophilic attack on the carbonyl carbon of the scissile peptide bond in the substrate ( ).	bind
50084	2	10959	5	13	NULL	NULL	NULL	water molecule	Chemical		bind					zinc	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_41_39497_s_169	12888578	A model for catalysis based on the metallopeptidase thermolysin proposes that the internal glutamic acid polarizes the zinc-bound water molecule for a nucleophilic attack on the carbonyl carbon of the scissile peptide bond in the substrate ( ).	bind
50085	3	10959	5	13	NULL	NULL	NULL			internal	polarize			glutamic acid		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_41_39497_s_169	12888578	A model for catalysis based on the metallopeptidase thermolysin proposes that the internal glutamic acid polarizes the zinc-bound water molecule for a nucleophilic attack on the carbonyl carbon of the scissile peptide bond in the substrate ( ).	bind
42196	1	10959	6	NULL	NULL	0	NULL	thermolysin	NULL		is a type of	NULL				metallopeptidase	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_41_39497_s_169	12888578	A model for catalysis based on the metallopeptidase thermolysin proposes that the internal glutamic acid polarizes the zinc-bound water molecule for a nucleophilic attack on the carbonyl carbon of the scissile peptide bond in the substrate ( ).	bind
42197	2	10959	6	NULL	NULL	0	NULL	zinc	NULL		bind	NULL				water molecule	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_41_39497_s_169	12888578	A model for catalysis based on the metallopeptidase thermolysin proposes that the internal glutamic acid polarizes the zinc-bound water molecule for a nucleophilic attack on the carbonyl carbon of the scissile peptide bond in the substrate ( ).	bind
42198	3	10959	6	NULL	NULL	0	NULL		NULL	internal	polarizes	NULL		glutamic acid		statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_41_39497_s_169	12888578	A model for catalysis based on the metallopeptidase thermolysin proposes that the internal glutamic acid polarizes the zinc-bound water molecule for a nucleophilic attack on the carbonyl carbon of the scissile peptide bond in the substrate ( ).	bind
50086	1	10960	5	13	NULL	NULL	NULL	ATP	Chemical		bind					Rho	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_41_26477_s_358	9756883	A Model for Catalysis-- Our model for the hydrolysis of three labeled ATP molecules bound to Rho when RNA and excess unlabeled ATP are added is shown in Scheme  1.	bind
42199	1	10960	6	NULL	NULL	0	NULL	ATP molecules	NULL		bind	NULL				Rho	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_41_26477_s_358	9756883	A Model for Catalysis-- Our model for the hydrolysis of three labeled ATP molecules bound to Rho when RNA and excess unlabeled ATP are added is shown in Scheme  1.	bind
50087	1	10961	5	13	NULL	NULL	NULL	GSH	GP		bind		covalently						Cys-32		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24798_s_92	10783391	A model for GSH covalently bound to Cys-32 as well as chemically reasonable water molecules and sulfate ions was built into sigmaA-weighted 2  F o    F c maps ( 30).	bind
50088	2	10961	5	13	NULL	NULL	NULL	GSH	GP		bind		covalently			water molecule	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24798_s_92	10783391	A model for GSH covalently bound to Cys-32 as well as chemically reasonable water molecules and sulfate ions was built into sigmaA-weighted 2  F o    F c maps ( 30).	bind
50089	3	10961	5	13	NULL	NULL	NULL	GSH	GP		bind		covalently			sulfate ions	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24798_s_92	10783391	A model for GSH covalently bound to Cys-32 as well as chemically reasonable water molecules and sulfate ions was built into sigmaA-weighted 2  F o    F c maps ( 30).	bind
42200	1	10961	6	NULL	NULL	0	NULL	GSH	NULL		bind	NULL	covalently				NULL		Cys-32		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24798_s_92	10783391	A model for GSH covalently bound to Cys-32 as well as chemically reasonable water molecules and sulfate ions was built into sigmaA-weighted 2  F o    F c maps ( 30).	bind
50524	2	10961	6	10	NULL	0	NULL	GSH	NULL		bind	NULL	covalently			water molecule	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24798_s_92	10783391	A model for GSH covalently bound to Cys-32 as well as chemically reasonable water molecules and sulfate ions was built into sigmaA-weighted 2  F o    F c maps ( 30).	bind
50526	3	10961	6	10	NULL	0	NULL	GSH	NULL		bind	NULL	covalently			sulfate ions	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24798_s_92	10783391	A model for GSH covalently bound to Cys-32 as well as chemically reasonable water molecules and sulfate ions was built into sigmaA-weighted 2  F o    F c maps ( 30).	bind
50090	1	10962	5	13	NULL	NULL	NULL	ISG15	GP		bind					UbE1L	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_29_27356_s_232	15917233	A Model For ISG15 Binding to UbE1L --	bind
42201	1	10962	6	NULL	NULL	0	NULL	ISG15	NULL		bind	NULL				UbE1L	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_27356_s_232	15917233	A Model For ISG15 Binding to UbE1L --	bind
50091	1	10963	5	13	NULL	NULL	NULL	G-protein	GP		bind		directly	betagamma subunit		Ca2+ channel	GP		alpha1B		NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_18_13_4883_s_153	9634554	A model for membrane-delimited voltage-dependent inhibition in which the G-protein betagamma subunit binds directly to the alpha1B Ca2+ channel has recently received experimental support (De Waard et al., 1997  ; Zamponi et al., 1997  ).	bind
42202	1	10963	6	10	NULL	0	NULL	G-protein 	NULL		bind	NULL	directly	betagamma subunit		 Ca2+ channel	NULL		alpha1B		NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_18_13_4883_s_153	9634554	A model for membrane-delimited voltage-dependent inhibition in which the G-protein betagamma subunit binds directly to the alpha1B Ca2+ channel has recently received experimental support (De Waard et al., 1997  ; Zamponi et al., 1997  ).	bind
50092	1	10964	5	13	NULL	NULL	NULL	N-CAM	GP		bind		homophilic	Ig I		N-CAM	GP		Ig V		NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_5_2592_s_16	9482931	A model for N-CAM homophilic binding has been proposed in which the Ig domains bind in a pairwise antiparallel manner such that Ig I binds Ig V, Ig II binds Ig IV, and Ig III binds Ig III ( 3).	bind
50093	2	10964	5	13	NULL	NULL	NULL	N-CAM	GP		bind		homophilic	Ig II		N-CAM	GP		Ig IV		NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_5_2592_s_16	9482931	A model for N-CAM homophilic binding has been proposed in which the Ig domains bind in a pairwise antiparallel manner such that Ig I binds Ig V, Ig II binds Ig IV, and Ig III binds Ig III ( 3).	bind
50094	3	10964	5	13	NULL	NULL	NULL	N-CAM	GP		bind		homophilic	Ig III		N-CAM	GP		Ig III		NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_5_2592_s_16	9482931	A model for N-CAM homophilic binding has been proposed in which the Ig domains bind in a pairwise antiparallel manner such that Ig I binds Ig V, Ig II binds Ig IV, and Ig III binds Ig III ( 3).	bind
42203	1	10964	6	10	NULL	0	NULL	N-CAM	NULL		bind	NULL	homophilic	Ig I		N-CAM	NULL		Ig V		NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_5_2592_s_16	9482931	A model for N-CAM homophilic binding has been proposed in which the Ig domains bind in a pairwise antiparallel manner such that Ig I binds Ig V, Ig II binds Ig IV, and Ig III binds Ig III ( 3).	bind
42204	2	10964	6	10	NULL	0	NULL	N-CAM	NULL		bind	NULL	homophilic	Ig II		N-CAM	NULL		Ig IV		NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_5_2592_s_16	9482931	A model for N-CAM homophilic binding has been proposed in which the Ig domains bind in a pairwise antiparallel manner such that Ig I binds Ig V, Ig II binds Ig IV, and Ig III binds Ig III ( 3).	bind
42205	3	10964	6	10	NULL	0	NULL	N-CAM	NULL		bind	NULL	homophilic	Ig III		N-CAM	NULL		Ig III		NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_5_2592_s_16	9482931	A model for N-CAM homophilic binding has been proposed in which the Ig domains bind in a pairwise antiparallel manner such that Ig I binds Ig V, Ig II binds Ig IV, and Ig III binds Ig III ( 3).	bind
50095	1	10965	5	13	NULL	NULL	NULL	Rad52 protein	GP		bind					RPA-ssDNA complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_35_31663_s_300	12077133	A model for presynaptic complex formation by Rad51 and Rad52 proteins and  RPA. Rad52 protein binds to RPA-ssDNA complex ( a) to form a Rad52-RPA-ssDNA nucleoprotein co-complex ( b).	bind
50097	2	10965	5	13	NULL	NULL	NULL	statement 1	Process		forms					Rad52-RPA-ssDNA nucleoprotein co-complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_35_31663_s_300	12077133	A model for presynaptic complex formation by Rad51 and Rad52 proteins and  RPA. Rad52 protein binds to RPA-ssDNA complex ( a) to form a Rad52-RPA-ssDNA nucleoprotein co-complex ( b).	bind
42206	1	10965	6	NULL	NULL	0	NULL	Rad52 protein	NULL		bind	NULL				RPA-ssDNA complex	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_35_31663_s_300	12077133	A model for presynaptic complex formation by Rad51 and Rad52 proteins and  RPA. Rad52 protein binds to RPA-ssDNA complex ( a) to form a Rad52-RPA-ssDNA nucleoprotein co-complex ( b).	bind
42207	2	10965	6	NULL	NULL	0	NULL	statement 1	NULL		forms a 	NULL				Rad52-RPA-ssDNA nucleoprotein co-complex	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_35_31663_s_300	12077133	A model for presynaptic complex formation by Rad51 and Rad52 proteins and  RPA. Rad52 protein binds to RPA-ssDNA complex ( a) to form a Rad52-RPA-ssDNA nucleoprotein co-complex ( b).	bind
50098	1	10966	5	13	NULL	NULL	NULL	Bas1p/Bas2p	GP		regulates					adenine	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_23_4665_s_236	11095676	A model for promoter-specific adenine regulation of the Bas1p/Bas2p couple.	bind
50099	2	10966	5	13	NULL	NULL	NULL	statement 1	Process		is specific to					promoter	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_23_4665_s_236	11095676	A model for promoter-specific adenine regulation of the Bas1p/Bas2p couple.	bind
42208	1	10966	6	10	NULL	0	NULL	Bas1p/Bas2p couple	NULL		regulate	NULL				adenine 	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_23_4665_s_236	11095676	A model for promoter-specific adenine regulation of the Bas1p/Bas2p couple.	bind
42209	2	10966	6	10	NULL	0	NULL	statement 1	NULL		is specific to	NULL				promoter	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_23_4665_s_236	11095676	A model for promoter-specific adenine regulation of the Bas1p/Bas2p couple.	bind
50100	1	10967	5	13	NULL	NULL	NULL	Rac1	GP		bind								IMD		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_2_240_s_202	15635447	A model for Rac1 binding  to the IMD can be readily derived by superimposing the IMD structure with the Rac1-arfaptin2  complex (  et al).	bind
42210	1	10967	6	10	NULL	0	NULL	Rac1	NULL		bind	NULL					NULL		IMD		NULL		NULL	NULL	NULL	NULL	gw70_embo_24_2_240_s_202	15635447	A model for Rac1 binding  to the IMD can be readily derived by superimposing the IMD structure with the Rac1-arfaptin2  complex (  et al).	bind
50101	1	10968	5	13	NULL	NULL	NULL	SDF-1	GP		bind					CXCR4	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_23_6996_s_193	9384579	A model for SDF-1 receptor [[ interactions        Based ]] on these results we propose a two site model for SDF-1 binding to CXCR4 (Figure  7).	bind
42211	1	10968	6	NULL	NULL	0	NULL	SDF-1	NULL		bind	NULL				CXCR4	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_16_23_6996_s_193	9384579	A model for SDF-1 receptor [[ interactions        Based ]] on these results we propose a two site model for SDF-1 binding to CXCR4 (Figure  7).	bind
50102	1	10969	5	13	NULL	NULL	NULL	Sm2DBD homodimer	GP		bind					target gene	GP				NULL		NULL	NULL	NULL	NULL	gw70_gene_366_2_303_s_48	16406405	A model for Sm2DBDs  bind to their target gene as a homodimer or heterodimer.	bind
50103	2	10969	5	13	NULL	NULL	NULL	Sm2DBD heterodimer	GP		bind					target gene	GP				NULL		NULL	NULL	NULL	NULL	gw70_gene_366_2_303_s_48	16406405	A model for Sm2DBDs  bind to their target gene as a homodimer or heterodimer.	bind
42213	1	10969	6	10	NULL	0	NULL	Sm2DBD homodimer	NULL		bind	NULL				target gene	NULL				NULL		NULL	NULL	NULL	NULL	gw70_gene_366_2_303_s_48	16406405	A model for Sm2DBDs  bind to their target gene as a homodimer or heterodimer.	bind
42214	2	10969	6	10	NULL	0	NULL	Sm2DBD heterodimer	NULL		bind	NULL				target gene	NULL				NULL		NULL	NULL	NULL	NULL	gw70_gene_366_2_303_s_48	16406405	A model for Sm2DBDs  bind to their target gene as a homodimer or heterodimer.	bind
50104	1	10970	5	13	NULL	NULL	NULL	Sm2DBD monomer	GP		bind					target gene	GP				NULL		NULL	NULL	NULL	NULL	gw70_gene_366_2_303_s_46	16406405	A model for Sm2DBDs bind to their target gene as monomer.	bind
42212	1	10970	6	10	NULL	0	NULL	Sm2DBD monomer	NULL		bind	NULL				target gene	NULL				NULL		NULL	NULL	NULL	NULL	gw70_gene_366_2_303_s_46	16406405	A model for Sm2DBDs bind to their target gene as monomer.	bind
50105	1	10971	5	13	NULL	NULL	NULL	TFIIB	GP		bind					TBP-DNA complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_1_34_s_302	9420329	A model for TFIIB binding to the TBP-DNA complex.	bind
42215	1	10971	6	NULL	NULL	0	NULL	TFIIB	NULL		bind	NULL				TBP-DNA complex	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_1_34_s_302	9420329	A model for TFIIB binding to the TBP-DNA complex.	bind
50106	1	10972	5	13	NULL	NULL	NULL	GATA-4	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_16_13752_s_319	11827958	A model for the  MAPK  regulation of transcription factor GATA-4 binding to   BNP  gene promoter by hypertrophic agonists.	bind
50107	2	10972	5	13	NULL	NULL	NULL	GATA-4	GP		bind					BNP gene	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_16_13752_s_319	11827958	A model for the  MAPK  regulation of transcription factor GATA-4 binding to   BNP  gene promoter by hypertrophic agonists.	bind
50108	3	10972	5	13	NULL	NULL	NULL	MAPK	GP		regulates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_16_13752_s_319	11827958	A model for the  MAPK  regulation of transcription factor GATA-4 binding to   BNP  gene promoter by hypertrophic agonists.	bind
42216	1	10972	6	NULL	NULL	0	NULL	GATA-4	NULL		bind	NULL				BNP gene	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_16_13752_s_319	11827958	A model for the  MAPK  regulation of transcription factor GATA-4 binding to   BNP  gene promoter by hypertrophic agonists.	bind
42217	2	10972	6	NULL	NULL	0	NULL	GATA-4	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_16_13752_s_319	11827958	A model for the  MAPK  regulation of transcription factor GATA-4 binding to   BNP  gene promoter by hypertrophic agonists.	bind
42218	3	10972	6	NULL	NULL	0	NULL	statement 1	NULL		is regulated by	NULL				MAPK	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_16_13752_s_319	11827958	A model for the  MAPK  regulation of transcription factor GATA-4 binding to   BNP  gene promoter by hypertrophic agonists.	bind
50109	1	10973	5	13	NULL	NULL	NULL	MT1-MMP	GP		bind			catalytic domain		TIMP-2	GP		N-terminus		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_52_41415_s_26	10998420	A model for the activation of pro-MMP-2 has been proposed in which the catalytic domain of MT1-MMP binds to the N-terminal portion of TIMP-2, leaving the negatively charged C-terminal region of TIMP-2 available for the binding of the hemopexin-like domain of pro-MMP-2 ( 12,  34-38).	bind
50110	2	10973	5	13	NULL	NULL	NULL	TIMP-2	GP		bind			negatively charged C-terminus		pro-MMP-2	GP		hemopexin-like domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_52_41415_s_26	10998420	A model for the activation of pro-MMP-2 has been proposed in which the catalytic domain of MT1-MMP binds to the N-terminal portion of TIMP-2, leaving the negatively charged C-terminal region of TIMP-2 available for the binding of the hemopexin-like domain of pro-MMP-2 ( 12,  34-38).	bind
42219	1	10973	6	NULL	NULL	0	NULL	MT1-MMP	NULL		bind	NULL		catalytic domain		TIMP-2	NULL		N-terminal 		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_52_41415_s_26	10998420	A model for the activation of pro-MMP-2 has been proposed in which the catalytic domain of MT1-MMP binds to the N-terminal portion of TIMP-2, leaving the negatively charged C-terminal region of TIMP-2 available for the binding of the hemopexin-like domain of pro-MMP-2 ( 12,  34-38).	bind
42220	2	10973	6	NULL	NULL	0	NULL	pro-MMP-2	NULL		bind	NULL		hemopexin-like domain		TIMP-2	NULL		negatively charged C-terminal region		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_52_41415_s_26	10998420	A model for the activation of pro-MMP-2 has been proposed in which the catalytic domain of MT1-MMP binds to the N-terminal portion of TIMP-2, leaving the negatively charged C-terminal region of TIMP-2 available for the binding of the hemopexin-like domain of pro-MMP-2 ( 12,  34-38).	bind
50111	1	10974	5	13	NULL	NULL	NULL	PS-I	GP		is a type of					reaction center	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_46_36250_s_149	10948201	A model for the binding of Fd to the PS-I reaction center is presented in Fig.  5.	bind
50112	2	10974	5	13	NULL	NULL	NULL	Fd	Chemical		bind					PS-I	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_46_36250_s_149	10948201	A model for the binding of Fd to the PS-I reaction center is presented in Fig.  5.	bind
42221	1	10974	6	NULL	NULL	0	NULL	Fd	NULL		bind	NULL				PS-I reaction center	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_46_36250_s_149	10948201	A model for the binding of Fd to the PS-I reaction center is presented in Fig.  5.	bind
50113	1	10975	5	13	NULL	NULL	NULL	unr	GP		bind					Apaf-1	GP			IRES	NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_3_757_s_226	12667457	A Model for the Binding of unr and nPTB to the Apaf-1 IRES during Ribosome Recruitment	bind
50114	2	10975	5	13	NULL	NULL	NULL	statement 1	Process		occurs during					ribosome	CellComponent	recruitment of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_3_757_s_226	12667457	A Model for the Binding of unr and nPTB to the Apaf-1 IRES during Ribosome Recruitment	bind
50115	3	10975	5	13	NULL	NULL	NULL	nPTB	GP		bind					Apaf-1	GP			IRES	NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_3_757_s_226	12667457	A Model for the Binding of unr and nPTB to the Apaf-1 IRES during Ribosome Recruitment	bind
50116	4	10975	5	13	NULL	NULL	NULL	statement 3	Process		occurs during					ribosome	CellComponent	recruitment of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_3_757_s_226	12667457	A Model for the Binding of unr and nPTB to the Apaf-1 IRES during Ribosome Recruitment	bind
42222	1	10975	6	NULL	NULL	0	NULL	unr	NULL		bind	NULL				Apaf-1	NULL			IRES	NULL		0	NULL	NULL	NULL	gw60_molcell_11_3_757_s_226	12667457	A Model for the Binding of unr and nPTB to the Apaf-1 IRES during Ribosome Recruitment	bind
42223	2	10975	6	NULL	NULL	0	NULL	nPTB	NULL		bind	NULL				Apaf-1	NULL			IRES	NULL		0	NULL	NULL	NULL	gw60_molcell_11_3_757_s_226	12667457	A Model for the Binding of unr and nPTB to the Apaf-1 IRES during Ribosome Recruitment	bind
42224	3	10975	6	NULL	NULL	0	NULL	statement 1	NULL		occurs during	NULL				ribosome	NULL	recruitment of			NULL		0	NULL	NULL	NULL	gw60_molcell_11_3_757_s_226	12667457	A Model for the Binding of unr and nPTB to the Apaf-1 IRES during Ribosome Recruitment	bind
42225	4	10975	6	NULL	NULL	0	NULL	statement 2	NULL		occurs during	NULL				ribosome	NULL	recruitment of			NULL		0	NULL	NULL	NULL	gw60_molcell_11_3_757_s_226	12667457	A Model for the Binding of unr and nPTB to the Apaf-1 IRES during Ribosome Recruitment	bind
50117	1	10976	5	13	NULL	NULL	NULL	MDM2	GP		degrades					p53	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_7288_s_206	9819415	A model for the degradation of p53 by MDM2.	bind
42226	1	10976	6	NULL	NULL	0	NULL	MDM2	NULL		degrades	NULL				p53	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_12_7288_s_206	9819415	A model for the degradation of p53 by MDM2.	bind
50118	1	10977	5	13	NULL	NULL	NULL	METH	Chemical		induce					DA responses	Process				NULL		NULL	NULL	NULL	NULL	gw70_jneurosci_24_9_2212_s_456	14999072	A model for the modulation by TNF-alpha of METH-induced DA responses.	bind
50119	2	10977	5	13	NULL	NULL	NULL	TNF-alpha	GP		modulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jneurosci_24_9_2212_s_456	14999072	A model for the modulation by TNF-alpha of METH-induced DA responses.	bind
42227	1	10977	6	NULL	NULL	0	NULL	METH	NULL		induces	NULL				DA responses	NULL				NULL		0	NULL	NULL	NULL	gw70_jneurosci_24_9_2212_s_456	14999072	A model for the modulation by TNF-alpha of METH-induced DA responses.	bind
42228	2	10977	6	10	NULL	0	NULL	TNF-alpha	NULL		modulates	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jneurosci_24_9_2212_s_456	14999072	A model for the modulation by TNF-alpha of METH-induced DA responses.	bind
50120	1	10978	5	13	NULL	NULL	NULL	m-xylene	Chemical		bind					XylR	GP		A domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_86_2_331_s_194	8706137	A Model for the Multimerization Cycle  of XylR at the UAS of the  Pu Promoter The series of events  that follow the release of intramolecular repression caused by  m-xylene binding to  the A domain of XylR are sketched in the figure as a  multimerization and demultimerization cycle driven by ATP.	bind
50121	2	10978	5	13	NULL	NULL	NULL	statement 1	Process		causes					intramolecular repression	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_86_2_331_s_194	8706137	A Model for the Multimerization Cycle  of XylR at the UAS of the  Pu Promoter The series of events  that follow the release of intramolecular repression caused by  m-xylene binding to  the A domain of XylR are sketched in the figure as a  multimerization and demultimerization cycle driven by ATP.	bind
42229	1	10978	6	NULL	NULL	0	NULL	m-xylene	NULL		bind	NULL				XylR	NULL		A domain		NULL		0	NULL	NULL	NULL	gw60_cell_86_2_331_s_194	8706137	A Model for the Multimerization Cycle  of XylR at the UAS of the  Pu Promoter The series of events  that follow the release of intramolecular repression caused by  m-xylene binding to  the A domain of XylR are sketched in the figure as a  multimerization and demultimerization cycle driven by ATP.	bind
50565	2	10978	6	10	NULL	0	NULL	statement 1	NULL		cause	NULL				intramolecular repression	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_86_2_331_s_194	8706137	A Model for the Multimerization Cycle  of XylR at the UAS of the  Pu Promoter The series of events  that follow the release of intramolecular repression caused by  m-xylene binding to  the A domain of XylR are sketched in the figure as a  multimerization and demultimerization cycle driven by ATP.	bind
50122	1	10979	5	13	NULL	NULL	NULL	PLC-delta1	GP		bind			pleckstrin homology domain		IP3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_37_34401_s_153	12097325	A model for the PIP2 head group was taken from the structure of the pleckstrin homology domain of PLC-delta1 bound to IP3 (Protein Data Bank code  1MAI) ( 65).	bind
42230	1	10979	6	NULL	NULL	0	NULL	PLC-delta1	NULL		bind	NULL		pleckstrin homology domain		IP3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_37_34401_s_153	12097325	A model for the PIP2 head group was taken from the structure of the pleckstrin homology domain of PLC-delta1 bound to IP3 (Protein Data Bank code  1MAI) ( 65).	bind
50123	1	10980	5	13	NULL	NULL	NULL	PAF	GP		bind					G protein-coupled seven transmembrane receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_5_3497_s_239	14617636	A model for the stimulation of separate pathways upon binding of PAF to its G protein-coupled  seven transmembrane receptor.	bind
42231	1	10980	6	NULL	NULL	0	NULL	PAF	NULL		bind	NULL				G protein-coupled seven transmembrane receptor	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_5_3497_s_239	14617636	A model for the stimulation of separate pathways upon binding of PAF to its G protein-coupled  seven transmembrane receptor.	bind
50124	1	10981	5	13	NULL	NULL	NULL	Frq1	GP	yeast	bind					Ca2+	Chemical	N-myristoylated			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49589_s_15	14512421	A model for the three-dimensional structure of  N-myristoylated Ca2+-bound yeast Frq1, based on analysis by NMR, is nearly superimposable ( ).	bind
42232	1	10981	6	10	NULL	0	NULL	Ca2+	NULL	N-myristoylated	bind	NULL				Frq1	NULL	yeast			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_49_49589_s_15	14512421	A model for the three-dimensional structure of  N-myristoylated Ca2+-bound yeast Frq1, based on analysis by NMR, is nearly superimposable ( ).	bind
50126	1	10982	5	13	NULL	NULL	NULL	thrombin	GP		is a type of					serine protease	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_7_1705_s_16	8601636	A model for thrombin receptor activation in which the  serine protease thrombin binds to an acidic hirudin-like domain and proteolytically cleaves the amino terminal exodomain of the thrombin receptor between Arg  41 and Ser42 ( 4)  has since been postulated.	bind
50127	2	10982	5	13	NULL	NULL	NULL	thrombin	GP		bind							acidic	hirudin-like domain		NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_7_1705_s_16	8601636	A model for thrombin receptor activation in which the  serine protease thrombin binds to an acidic hirudin-like domain and proteolytically cleaves the amino terminal exodomain of the thrombin receptor between Arg  41 and Ser42 ( 4)  has since been postulated.	bind
50128	3	10982	5	13	NULL	NULL	NULL	statement 1	GP		cleaves		proteolytically			thrombin receptor	GP		amino terminal exodomain;;between Arg 41 and Ser42		NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_97_7_1705_s_16	8601636	A model for thrombin receptor activation in which the  serine protease thrombin binds to an acidic hirudin-like domain and proteolytically cleaves the amino terminal exodomain of the thrombin receptor between Arg  41 and Ser42 ( 4)  has since been postulated.	bind
42233	1	10982	6	NULL	NULL	0	NULL	thrombin	NULL		is a type of	NULL				serine protease	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_97_7_1705_s_16	8601636	A model for thrombin receptor activation in which the  serine protease thrombin binds to an acidic hirudin-like domain and proteolytically cleaves the amino terminal exodomain of the thrombin receptor between Arg  41 and Ser42 ( 4)  has since been postulated.	bind
42234	2	10982	6	NULL	NULL	0	NULL	thrombin	NULL		bind	NULL					NULL	acidic	hirudin-like domain 		NULL		0	NULL	NULL	NULL	gw60_jclininvest_97_7_1705_s_16	8601636	A model for thrombin receptor activation in which the  serine protease thrombin binds to an acidic hirudin-like domain and proteolytically cleaves the amino terminal exodomain of the thrombin receptor between Arg  41 and Ser42 ( 4)  has since been postulated.	bind
42235	3	10982	6	NULL	NULL	0	NULL	thrombin	NULL		cleaves	NULL	proteolytically			thrombin receptor	NULL		amino terminal exodomain;; between Arg 41 and Ser42		NULL		0	NULL	NULL	NULL	gw60_jclininvest_97_7_1705_s_16	8601636	A model for thrombin receptor activation in which the  serine protease thrombin binds to an acidic hirudin-like domain and proteolytically cleaves the amino terminal exodomain of the thrombin receptor between Arg  41 and Ser42 ( 4)  has since been postulated.	bind
50133	1	10983	5	13	NULL	NULL	NULL	Gpb1/2	GP		bind					Gpa2	GP		N-terminus amino acids 1 - 45		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4557_s_321	16030250	A model governing how the kelch Gpb1/2 subunits control Gpa2 is that Gpb1/2 bind to the Gpa2 N-terminal region spanning amino acids 1 - 45 and occlude binding of the Gpr1 C-terminal tail to the first fifteen amino acids of Gpa2 ( Figure 9).	bind
50134	2	10983	5	13	NULL	NULL	NULL	Gpr1	GP		bind			C-terminal tail 		Gpa2	GP		first fifteen amino acids of		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4557_s_321	16030250	A model governing how the kelch Gpb1/2 subunits control Gpa2 is that Gpb1/2 bind to the Gpa2 N-terminal region spanning amino acids 1 - 45 and occlude binding of the Gpr1 C-terminal tail to the first fifteen amino acids of Gpa2 ( Figure 9).	bind
50135	3	10983	5	13	NULL	NULL	NULL	statement 1	Process		occlude					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4557_s_321	16030250	A model governing how the kelch Gpb1/2 subunits control Gpa2 is that Gpb1/2 bind to the Gpa2 N-terminal region spanning amino acids 1 - 45 and occlude binding of the Gpr1 C-terminal tail to the first fifteen amino acids of Gpa2 ( Figure 9).	bind
42236	1	10983	6	NULL	NULL	0	NULL	Gpb1/2	NULL		bind	NULL				Gpa2	NULL		N-terminal region;; amino acid 1 to 45		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4557_s_321	16030250	A model governing how the kelch Gpb1/2 subunits control Gpa2 is that Gpb1/2 bind to the Gpa2 N-terminal region spanning amino acids 1 - 45 and occlude binding of the Gpr1 C-terminal tail to the first fifteen amino acids of Gpa2 ( Figure 9).	bind
42237	2	10983	6	NULL	NULL	0	NULL	Gpr1	NULL		bind	NULL		C-terminal tail		Gpa2	NULL		first fifteen amino acid		NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4557_s_321	16030250	A model governing how the kelch Gpb1/2 subunits control Gpa2 is that Gpb1/2 bind to the Gpa2 N-terminal region spanning amino acids 1 - 45 and occlude binding of the Gpr1 C-terminal tail to the first fifteen amino acids of Gpa2 ( Figure 9).	bind
42238	3	10983	6	NULL	NULL	0	NULL	statement 1	NULL		occlude	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4557_s_321	16030250	A model governing how the kelch Gpb1/2 subunits control Gpa2 is that Gpb1/2 bind to the Gpa2 N-terminal region spanning amino acids 1 - 45 and occlude binding of the Gpr1 C-terminal tail to the first fifteen amino acids of Gpa2 ( Figure 9).	bind
50137	1	10984	5	13	NULL	NULL	NULL	MBP	GP	unfolded form of	bind					SecB	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_40_38247_s_29	12829711	A model has been proposed for the interaction of SecB and MBP: an unfolded form of MBP binds to SecB and is in equilibrium with unbound form.	bind
50138	2	10984	5	13	NULL	NULL	NULL	statement 1	Process		is in equilibrium with					MBP	GP	unbound form of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_40_38247_s_29	12829711	A model has been proposed for the interaction of SecB and MBP: an unfolded form of MBP binds to SecB and is in equilibrium with unbound form.	bind
42239	1	10984	6	NULL	NULL	0	NULL	SecB	NULL		interacts with	NULL				MBP	NULL	unfolded			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_40_38247_s_29	12829711	A model has been proposed for the interaction of SecB and MBP: an unfolded form of MBP binds to SecB and is in equilibrium with unbound form.	bind
58415	2	10984	6	10	NULL	0	NULL	statement 1			is in equilibrium with					MBP		unbound form of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_40_38247_s_29	12829711	A model has been proposed for the interaction of SecB and MBP: an unfolded form of MBP binds to SecB and is in equilibrium with unbound form.	bind
50129	1	10985	5	13	NULL	NULL	NULL	syndecan 4	GP		bind		low affinity						cysteine-rich domain		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_2_861_s_26	15574885	A model has been proposed in which initial low-affinity binding of the cysteine-rich domain by syndecan 4 triggers a conformational change of ADAM12- cys, allowing its binding to integrins (Iba  et al., 2000 ).	bind
50130	2	10985	5	13	NULL	NULL	NULL	statement 1	Process		triggers					ADAM12	GP	conformational change of	cys		NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_2_861_s_26	15574885	A model has been proposed in which initial low-affinity binding of the cysteine-rich domain by syndecan 4 triggers a conformational change of ADAM12- cys, allowing its binding to integrins (Iba  et al., 2000 ).	bind
50131	3	10985	5	13	NULL	NULL	NULL	ADAM12	GP		bind			cys		integrins 	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_2_861_s_26	15574885	A model has been proposed in which initial low-affinity binding of the cysteine-rich domain by syndecan 4 triggers a conformational change of ADAM12- cys, allowing its binding to integrins (Iba  et al., 2000 ).	bind
50132	4	10985	5	13	NULL	NULL	NULL	statement 2	Process		allows					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_2_861_s_26	15574885	A model has been proposed in which initial low-affinity binding of the cysteine-rich domain by syndecan 4 triggers a conformational change of ADAM12- cys, allowing its binding to integrins (Iba  et al., 2000 ).	bind
42240	1	10985	6	NULL	NULL	0	NULL		NULL		bind	NULL	low affinity	cysteine-rich domain		syndecan-4	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_2_861_s_26	15574885	A model has been proposed in which initial low-affinity binding of the cysteine-rich domain by syndecan 4 triggers a conformational change of ADAM12- cys, allowing its binding to integrins (Iba  et al., 2000 ).	bind
42241	2	10985	6	NULL	NULL	0	NULL	statement 1	NULL		triggers	NULL				ADAM12	NULL	conformational change of	Cys		NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_2_861_s_26	15574885	A model has been proposed in which initial low-affinity binding of the cysteine-rich domain by syndecan 4 triggers a conformational change of ADAM12- cys, allowing its binding to integrins (Iba  et al., 2000 ).	bind
42242	3	10985	6	NULL	NULL	0	NULL	ADAM12	NULL		bind	NULL		cys		integrin	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_2_861_s_26	15574885	A model has been proposed in which initial low-affinity binding of the cysteine-rich domain by syndecan 4 triggers a conformational change of ADAM12- cys, allowing its binding to integrins (Iba  et al., 2000 ).	bind
42243	4	10985	6	NULL	NULL	0	NULL	statement 2	NULL		leads to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_2_861_s_26	15574885	A model has been proposed in which initial low-affinity binding of the cysteine-rich domain by syndecan 4 triggers a conformational change of ADAM12- cys, allowing its binding to integrins (Iba  et al., 2000 ).	bind
50136	1	10986	5	13	NULL	NULL	NULL	SipA	GP		bind					actin monomers	GP	consecutive			NULL		NULL	NULL	NULL	NULL	gw60_annurevcelldevbiol_17_0_53_s_196	11687484	A model has been proposed in which SipA binds two consecutive actin monomers across the double-stranded right-handed helix in both of its faces ( Mitra et al. 2000) ( Figure 4).	bind
50572	2	10986	5	13	NULL	NULL	NULL	statement 1	Process		occur across					double-stranded right-handed helix	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_annurevcelldevbiol_17_0_53_s_196	11687484	A model has been proposed in which SipA binds two consecutive actin monomers across the double-stranded right-handed helix in both of its faces ( Mitra et al. 2000) ( Figure 4).	bind
42244	1	10986	6	NULL	NULL	0	NULL	SipA	NULL		bind	NULL				actin monomer	NULL				NULL		0	NULL	NULL	NULL	gw60_annurevcelldevbiol_17_0_53_s_196	11687484	A model has been proposed in which SipA binds two consecutive actin monomers across the double-stranded right-handed helix in both of its faces ( Mitra et al. 2000) ( Figure 4).	bind
42245	2	10986	6	10	NULL	0	NULL	statement 1	NULL		occurs across	NULL				double-stranded right-handed helix	NULL				NULL		NULL	NULL	NULL	NULL	gw60_annurevcelldevbiol_17_0_53_s_196	11687484	A model has been proposed in which SipA binds two consecutive actin monomers across the double-stranded right-handed helix in both of its faces ( Mitra et al. 2000) ( Figure 4).	bind
50139	1	10987	5	13	NULL	NULL	NULL	S1P	GP		bind					EDG receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_8_s_136	12069805	A model has been proposed that implicates LPPs in S1P signal termination at EDG receptors [ 1, whereby S1P binding to EDG receptors stimulates protein kinases, which then both transmit movement signals and phosphorylate and activate the putative signal terminator phosphatase [ 1.	bind
50140	2	10987	5	13	NULL	NULL	NULL	statement 1	Process		stimulates					protein kinases	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_8_s_136	12069805	A model has been proposed that implicates LPPs in S1P signal termination at EDG receptors [ 1, whereby S1P binding to EDG receptors stimulates protein kinases, which then both transmit movement signals and phosphorylate and activate the putative signal terminator phosphatase [ 1.	bind
50141	3	10987	5	13	NULL	NULL	NULL	statement 1	Process		transmit					movement signals	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_8_s_136	12069805	A model has been proposed that implicates LPPs in S1P signal termination at EDG receptors [ 1, whereby S1P binding to EDG receptors stimulates protein kinases, which then both transmit movement signals and phosphorylate and activate the putative signal terminator phosphatase [ 1.	bind
50142	4	10987	5	13	NULL	NULL	NULL	statement 1	Process		phosphorylates					signal terminator phosphatase	GP	putative			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_8_s_136	12069805	A model has been proposed that implicates LPPs in S1P signal termination at EDG receptors [ 1, whereby S1P binding to EDG receptors stimulates protein kinases, which then both transmit movement signals and phosphorylate and activate the putative signal terminator phosphatase [ 1.	bind
50143	5	10987	5	13	NULL	NULL	NULL	statement 1	Process		activates					signal terminator phosphatase	GP	putative			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_8_s_136	12069805	A model has been proposed that implicates LPPs in S1P signal termination at EDG receptors [ 1, whereby S1P binding to EDG receptors stimulates protein kinases, which then both transmit movement signals and phosphorylate and activate the putative signal terminator phosphatase [ 1.	bind
42246	1	10987	6	NULL	NULL	0	NULL	S1P	NULL		bind	NULL				EDG receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_8_s_136	12069805	A model has been proposed that implicates LPPs in S1P signal termination at EDG receptors [ 1, whereby S1P binding to EDG receptors stimulates protein kinases, which then both transmit movement signals and phosphorylate and activate the putative signal terminator phosphatase [ 1.	bind
42247	2	10987	6	NULL	NULL	0	NULL	statement 1	NULL		stimulates	NULL				protein kinases	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_8_s_136	12069805	A model has been proposed that implicates LPPs in S1P signal termination at EDG receptors [ 1, whereby S1P binding to EDG receptors stimulates protein kinases, which then both transmit movement signals and phosphorylate and activate the putative signal terminator phosphatase [ 1.	bind
42248	3	10987	6	10	NULL	0	NULL	statement 1	NULL		phosphorylates	NULL				signal terminator phosphatase	NULL	putative			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_8_s_136	12069805	A model has been proposed that implicates LPPs in S1P signal termination at EDG receptors [ 1, whereby S1P binding to EDG receptors stimulates protein kinases, which then both transmit movement signals and phosphorylate and activate the putative signal terminator phosphatase [ 1.	bind
42249	4	10987	6	10	NULL	0	NULL	statement 1	NULL		activates	NULL				signal terminator phosphatase	NULL	putative			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_8_s_136	12069805	A model has been proposed that implicates LPPs in S1P signal termination at EDG receptors [ 1, whereby S1P binding to EDG receptors stimulates protein kinases, which then both transmit movement signals and phosphorylate and activate the putative signal terminator phosphatase [ 1.	bind
42250	5	10987	6	10	NULL	0	NULL	statement 1	NULL		transmit	NULL				movement signals	NULL				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_8_s_136	12069805	A model has been proposed that implicates LPPs in S1P signal termination at EDG receptors [ 1, whereby S1P binding to EDG receptors stimulates protein kinases, which then both transmit movement signals and phosphorylate and activate the putative signal terminator phosphatase [ 1.	bind
50144	1	10989	5	13	NULL	NULL	NULL	FGF2	GP		complex with					FGFR1	GP		ligand binding domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_101_4_413_s_11	10830168	A model has emerged from the recent crystal structure of  FGF2 complexed with the ligand binding domain of FGFR1 to explain how  FGFs in concert with heparin induce FGFR dimerization and activation (Plotnikov et  al., 1999   ).	bind
50145	2	10989	5	13	NULL	NULL	NULL	FGFs	GP		induce					FGFR	GP	dimerization of			NULL		NULL	NULL	NULL	NULL	gw60_cell_101_4_413_s_11	10830168	A model has emerged from the recent crystal structure of  FGF2 complexed with the ligand binding domain of FGFR1 to explain how  FGFs in concert with heparin induce FGFR dimerization and activation (Plotnikov et  al., 1999   ).	bind
50146	3	10989	5	13	NULL	NULL	NULL	statement 2	Process		in concert with					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_101_4_413_s_11	10830168	A model has emerged from the recent crystal structure of  FGF2 complexed with the ligand binding domain of FGFR1 to explain how  FGFs in concert with heparin induce FGFR dimerization and activation (Plotnikov et  al., 1999   ).	bind
50147	4	10989	5	13	NULL	NULL	NULL	FGFs	GP		induce					FGFR	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_cell_101_4_413_s_11	10830168	A model has emerged from the recent crystal structure of  FGF2 complexed with the ligand binding domain of FGFR1 to explain how  FGFs in concert with heparin induce FGFR dimerization and activation (Plotnikov et  al., 1999   ).	bind
50148	5	10989	5	13	NULL	NULL	NULL	statement 4	Process		in concert with					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_101_4_413_s_11	10830168	A model has emerged from the recent crystal structure of  FGF2 complexed with the ligand binding domain of FGFR1 to explain how  FGFs in concert with heparin induce FGFR dimerization and activation (Plotnikov et  al., 1999   ).	bind
42251	1	10989	6	10	NULL	0	NULL	FGF2	NULL		complex with	NULL				FGFR1	NULL		ligand binding domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_101_4_413_s_11	10830168	A model has emerged from the recent crystal structure of  FGF2 complexed with the ligand binding domain of FGFR1 to explain how  FGFs in concert with heparin induce FGFR dimerization and activation (Plotnikov et  al., 1999   ).	bind
42252	2	10989	6	NULL	NULL	0	NULL	FGF	NULL		induce	NULL				FGFR	NULL	dimerization of			NULL		0	NULL	NULL	NULL	gw60_cell_101_4_413_s_11	10830168	A model has emerged from the recent crystal structure of  FGF2 complexed with the ligand binding domain of FGFR1 to explain how  FGFs in concert with heparin induce FGFR dimerization and activation (Plotnikov et  al., 1999   ).	bind
42253	3	10989	6	NULL	NULL	0	NULL	statement 2	NULL		occurs in concert with	NULL				heparin	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_101_4_413_s_11	10830168	A model has emerged from the recent crystal structure of  FGF2 complexed with the ligand binding domain of FGFR1 to explain how  FGFs in concert with heparin induce FGFR dimerization and activation (Plotnikov et  al., 1999   ).	bind
42254	4	10989	6	NULL	NULL	0	NULL	FGF	NULL		induce	NULL				FGFR	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_cell_101_4_413_s_11	10830168	A model has emerged from the recent crystal structure of  FGF2 complexed with the ligand binding domain of FGFR1 to explain how  FGFs in concert with heparin induce FGFR dimerization and activation (Plotnikov et  al., 1999   ).	bind
42255	5	10989	6	NULL	NULL	0	NULL	statement 4	NULL		occurs in concert with	NULL				heparin	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_101_4_413_s_11	10830168	A model has emerged from the recent crystal structure of  FGF2 complexed with the ligand binding domain of FGFR1 to explain how  FGFs in concert with heparin induce FGFR dimerization and activation (Plotnikov et  al., 1999   ).	bind
50149	1	10990	5	13	NULL	NULL	NULL	IkappaBbeta	GP	newly synthesized;;unphosphorylated	bind					NF-kappaB	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_477_s_234	9418895	A model has recently been proposed ( 65), in which after the stimulus-induced degradation of both IkappaBs, the binding of the newly synthesized unphosphorylated IkappaBbeta to NF-kappaB blocks the inhibitory effect of the newly synthesized IkappaBalpha.	bind
50150	2	10990	5	13	NULL	NULL	NULL	statement 1	Process		blocks					IkappaBalpha	GP	inhibitory effect of;;newly synthesized			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_477_s_234	9418895	A model has recently been proposed ( 65), in which after the stimulus-induced degradation of both IkappaBs, the binding of the newly synthesized unphosphorylated IkappaBbeta to NF-kappaB blocks the inhibitory effect of the newly synthesized IkappaBalpha.	bind
50151	3	10990	5	13	NULL	NULL	NULL	stimulus	Process		induce					IkappaBs	GP	degradation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_477_s_234	9418895	A model has recently been proposed ( 65), in which after the stimulus-induced degradation of both IkappaBs, the binding of the newly synthesized unphosphorylated IkappaBbeta to NF-kappaB blocks the inhibitory effect of the newly synthesized IkappaBalpha.	bind
50573	4	10990	5	13	NULL	NULL	NULL	statement 2	Process		occurs after					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_477_s_234	9418895	A model has recently been proposed ( 65), in which after the stimulus-induced degradation of both IkappaBs, the binding of the newly synthesized unphosphorylated IkappaBbeta to NF-kappaB blocks the inhibitory effect of the newly synthesized IkappaBalpha.	bind
42256	1	10990	6	NULL	NULL	0	NULL	IkappaBbeta	NULL	newly synthesized;; unphosphorylated	bind	NULL				NF-kappaB	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_477_s_234	9418895	A model has recently been proposed ( 65), in which after the stimulus-induced degradation of both IkappaBs, the binding of the newly synthesized unphosphorylated IkappaBbeta to NF-kappaB blocks the inhibitory effect of the newly synthesized IkappaBalpha.	bind
42257	2	10990	6	10	NULL	0	NULL	statement 1	NULL		blocks	NULL				IkappaBalpha	NULL	inhibitory effect of ;;newly synthesized			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_477_s_234	9418895	A model has recently been proposed ( 65), in which after the stimulus-induced degradation of both IkappaBs, the binding of the newly synthesized unphosphorylated IkappaBbeta to NF-kappaB blocks the inhibitory effect of the newly synthesized IkappaBalpha.	bind
42258	3	10990	6	10	NULL	0	NULL	stimulus	NULL		induce	NULL				IkappaBs	NULL	degradation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_477_s_234	9418895	A model has recently been proposed ( 65), in which after the stimulus-induced degradation of both IkappaBs, the binding of the newly synthesized unphosphorylated IkappaBbeta to NF-kappaB blocks the inhibitory effect of the newly synthesized IkappaBalpha.	bind
50574	4	10990	6	10	NULL	0	NULL	statement 2	NULL		occurs after	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_477_s_234	9418895	A model has recently been proposed ( 65), in which after the stimulus-induced degradation of both IkappaBs, the binding of the newly synthesized unphosphorylated IkappaBbeta to NF-kappaB blocks the inhibitory effect of the newly synthesized IkappaBalpha.	bind
50152	1	10991	5	13	NULL	NULL	NULL	SM	GP		bind					pre-mRNA	NucleicAcid			3' terminus	NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_15_8852_s_232	9671768	A model in which SM binds pre-mRNA at the 3' terminus is consistent with the negative effect of SM on intron-containing transcripts.	bind
50575	2	10991	5	13	NULL	NULL	NULL	SM	GP		effect		negatively			intron-containing transcripts	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_15_8852_s_232	9671768	A model in which SM binds pre-mRNA at the 3' terminus is consistent with the negative effect of SM on intron-containing transcripts.	bind
42259	1	10991	6	10	NULL	0	NULL	SM			bind					pre-mRNA				3' terminus	NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_15_8852_s_232	9671768	A model in which SM binds pre-mRNA at the 3' terminus is consistent with the negative effect of SM on intron-containing transcripts.	bind
42260	2	10991	6	10	NULL	0	NULL	SM 	NULL		effect	NULL	negatively			intron-containing transcripts	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_15_8852_s_232	9671768	A model in which SM binds pre-mRNA at the 3' terminus is consistent with the negative effect of SM on intron-containing transcripts.	bind
50153	1	10992	5	13	NULL	NULL	NULL	gp31	GP		bind					GroEL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34075_s_344	9852065	A model in which the binding of gp31 to GroEL creates a larger folding cavity than when GroES is bound to GroEL could also explain the GroEL-gp31-specific requirement.	bind
50154	2	10992	5	13	NULL	NULL	NULL	GroES	GP		bind					GroEL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34075_s_344	9852065	A model in which the binding of gp31 to GroEL creates a larger folding cavity than when GroES is bound to GroEL could also explain the GroEL-gp31-specific requirement.	bind
50155	3	10992	5	13	NULL	NULL	NULL	statement 1	Process		creates					folding cavity	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34075_s_344	9852065	A model in which the binding of gp31 to GroEL creates a larger folding cavity than when GroES is bound to GroEL could also explain the GroEL-gp31-specific requirement.	bind
50156	4	10992	5	13	NULL	NULL	NULL	statement 2	Process		creates					folding cavity	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34075_s_344	9852065	A model in which the binding of gp31 to GroEL creates a larger folding cavity than when GroES is bound to GroEL could also explain the GroEL-gp31-specific requirement.	bind
50157	5	10992	5	13	NULL	NULL	NULL	statement 3	Process		is larger than					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34075_s_344	9852065	A model in which the binding of gp31 to GroEL creates a larger folding cavity than when GroES is bound to GroEL could also explain the GroEL-gp31-specific requirement.	bind
42261	1	10992	6	NULL	NULL	0	NULL	gp31	NULL		bind	NULL				GroEL	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_51_34075_s_344	9852065	A model in which the binding of gp31 to GroEL creates a larger folding cavity than when GroES is bound to GroEL could also explain the GroEL-gp31-specific requirement.	bind
42262	2	10992	6	NULL	NULL	0	NULL	GroES	NULL		bind	NULL				GroEL	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_51_34075_s_344	9852065	A model in which the binding of gp31 to GroEL creates a larger folding cavity than when GroES is bound to GroEL could also explain the GroEL-gp31-specific requirement.	bind
50576	3	10992	6	10	NULL	0	NULL	statement 1	NULL		creates	NULL				folding cavity	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_51_34075_s_344	9852065	A model in which the binding of gp31 to GroEL creates a larger folding cavity than when GroES is bound to GroEL could also explain the GroEL-gp31-specific requirement.	bind
50577	4	10992	6	10	NULL	0	NULL	statement 2	NULL		creates	NULL				folding cavity	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_51_34075_s_344	9852065	A model in which the binding of gp31 to GroEL creates a larger folding cavity than when GroES is bound to GroEL could also explain the GroEL-gp31-specific requirement.	bind
50578	5	10992	6	10	NULL	0	NULL	statement 3	NULL		is larger than	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_51_34075_s_344	9852065	A model in which the binding of gp31 to GroEL creates a larger folding cavity than when GroES is bound to GroEL could also explain the GroEL-gp31-specific requirement.	bind
50159	1	10994	5	13	NULL	NULL	NULL	Rac1	GP		bind			effector region		p67 phox	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_30_18834_s_13	9228059	A model is discussed in which the Rac1 effector region binds to p67 phox, the C terminus binds to the membrane, and the insert region interacts with a different protein component, possibly cytochrome  b558.	bind
50160	2	10994	5	13	NULL	NULL	NULL	Rac1	GP		bind			C terminus		membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_30_18834_s_13	9228059	A model is discussed in which the Rac1 effector region binds to p67 phox, the C terminus binds to the membrane, and the insert region interacts with a different protein component, possibly cytochrome  b558.	bind
50161	3	10994	5	13	NULL	NULL	NULL	Rac1	GP		interacts with		possibly	insert region		cytochrome b558	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_30_18834_s_13	9228059	A model is discussed in which the Rac1 effector region binds to p67 phox, the C terminus binds to the membrane, and the insert region interacts with a different protein component, possibly cytochrome  b558.	bind
42263	1	10994	6	NULL	NULL	0	NULL	Rac1	NULL		bind	NULL		effector region		p67 phox	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_30_18834_s_13	9228059	A model is discussed in which the Rac1 effector region binds to p67 phox, the C terminus binds to the membrane, and the insert region interacts with a different protein component, possibly cytochrome  b558.	bind
42264	2	10994	6	NULL	NULL	0	NULL	Rac1	NULL		bind	NULL		C terminus		membrane	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_30_18834_s_13	9228059	A model is discussed in which the Rac1 effector region binds to p67 phox, the C terminus binds to the membrane, and the insert region interacts with a different protein component, possibly cytochrome  b558.	bind
42265	3	10994	6	NULL	NULL	0	NULL	Rac1	NULL		interacts with	NULL	possibly	insert region		cytochrome b558	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_30_18834_s_13	9228059	A model is discussed in which the Rac1 effector region binds to p67 phox, the C terminus binds to the membrane, and the insert region interacts with a different protein component, possibly cytochrome  b558.	bind
50162	1	10995	5	13	NULL	NULL	NULL	TSU	GP		bind		sequence specifically			extracts containing STAT1	GP				NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_60_1_23_s_234	9858482	A model is proposed in  Figure 8 that takes into account the observed reduction in STAT1 translocation in TSU stable transfectants as well as the saturable and sequence-specific binding of TSU and small loop-loop model RNA to extracts containing STAT1.	bind
50163	2	10995	5	13	NULL	NULL	NULL	small loop-loop model RNA	NucleicAcid		bind		sequence specifically			extracts containing STAT1	GP				NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_60_1_23_s_234	9858482	A model is proposed in  Figure 8 that takes into account the observed reduction in STAT1 translocation in TSU stable transfectants as well as the saturable and sequence-specific binding of TSU and small loop-loop model RNA to extracts containing STAT1.	bind
42501	1	10995	6	NULL	NULL	0	NULL	TSU	NULL		bind	NULL	sequence specifically			extracts containing STAT1	NULL				NULL		0	NULL	NULL	NULL	gw60_biolreprod_60_1_23_s_234	9858482	A model is proposed in  Figure 8 that takes into account the observed reduction in STAT1 translocation in TSU stable transfectants as well as the saturable and sequence-specific binding of TSU and small loop-loop model RNA to extracts containing STAT1.	bind
42502	2	10995	6	NULL	NULL	0	NULL	small loop-loop model RNA	NULL		bind	NULL	sequence specifically			extracts containing STAT1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_60_1_23_s_234	9858482	A model is proposed in  Figure 8 that takes into account the observed reduction in STAT1 translocation in TSU stable transfectants as well as the saturable and sequence-specific binding of TSU and small loop-loop model RNA to extracts containing STAT1.	bind
50164	1	10996	5	13	NULL	NULL	NULL	TorI	GP		bind					TorR	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_25_9423_s_32	15197250	A model is proposed in which binding of TorI to TorR could prevent RNA polymerase recruitment to the  torC promoter.	bind
50165	2	10996	5	13	NULL	NULL	NULL	RNA polymerase	GP		is recruited to					torC	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_25_9423_s_32	15197250	A model is proposed in which binding of TorI to TorR could prevent RNA polymerase recruitment to the  torC promoter.	bind
50166	3	10996	5	13	NULL	NULL	NULL	statement 1	Process		prevents					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_25_9423_s_32	15197250	A model is proposed in which binding of TorI to TorR could prevent RNA polymerase recruitment to the  torC promoter.	bind
42266	1	10996	6	NULL	NULL	0	NULL	TorI	NULL		bind	NULL				TorR	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_101_25_9423_s_32	15197250	A model is proposed in which binding of TorI to TorR could prevent RNA polymerase recruitment to the  torC promoter.	bind
42267	2	10996	6	NULL	NULL	0	NULL	RNA polymerase 	NULL		is recruited to	NULL				torC 	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_pnas_101_25_9423_s_32	15197250	A model is proposed in which binding of TorI to TorR could prevent RNA polymerase recruitment to the  torC promoter.	bind
42268	3	10996	6	NULL	NULL	0	NULL	statement 1	NULL		prevents	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_101_25_9423_s_32	15197250	A model is proposed in which binding of TorI to TorR could prevent RNA polymerase recruitment to the  torC promoter.	bind
50167	1	10997	5	13	NULL	NULL	NULL	RNA-2	NucleicAcid		bind		directly			RNA-1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5378_829_s_10	9694655	A model is proposed in which direct binding of RNA-2 to RNA-1 trans-activates sgRNA synthesis.	bind
50168	2	10997	5	13	NULL	NULL	NULL	statement 1	Process		trans-activates					sgRNA	NucleicAcid	synthesis of			NULL		NULL	NULL	NULL	NULL	gw60_science_281_5378_829_s_10	9694655	A model is proposed in which direct binding of RNA-2 to RNA-1 trans-activates sgRNA synthesis.	bind
42269	1	10997	6	NULL	NULL	0	NULL	RNA-2	NULL		bind	NULL	directly			RNA-1	NULL				NULL		0	NULL	NULL	NULL	gw60_science_281_5378_829_s_10	9694655	A model is proposed in which direct binding of RNA-2 to RNA-1 trans-activates sgRNA synthesis.	bind
42270	2	10997	6	10	NULL	0	NULL	statement 1	NULL		trans-activates	NULL				sgRNA	NULL	synthesis of			NULL		NULL	NULL	NULL	NULL	gw60_science_281_5378_829_s_10	9694655	A model is proposed in which direct binding of RNA-2 to RNA-1 trans-activates sgRNA synthesis.	bind
50169	1	10998	5	13	NULL	NULL	NULL	IF1	GP		bind					F1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_9927_s_48	15640141	A model is proposed where the rate of IF1 binding to F1 is controlled by changes in the conformation of the IF1 binding site on F1, which depends on the catalytic state of the enzyme.	bind
50170	2	10998	5	13	NULL	NULL	NULL	statement 1	Process	rate of	is controlled by					F1	GP	changes in conformation of	IF1 binding site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_9927_s_48	15640141	A model is proposed where the rate of IF1 binding to F1 is controlled by changes in the conformation of the IF1 binding site on F1, which depends on the catalytic state of the enzyme.	bind
50171	3	10998	5	13	NULL	NULL	NULL	F1	GP	changes in conformation of	depends on			IF1 binding site		enzyme	GP	catalytic state of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_11_9927_s_48	15640141	A model is proposed where the rate of IF1 binding to F1 is controlled by changes in the conformation of the IF1 binding site on F1, which depends on the catalytic state of the enzyme.	bind
42271	1	10998	6	NULL	NULL	0	NULL	IF1	NULL		bind	NULL				F1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_11_9927_s_48	15640141	A model is proposed where the rate of IF1 binding to F1 is controlled by changes in the conformation of the IF1 binding site on F1, which depends on the catalytic state of the enzyme.	bind
42503	2	10998	6	NULL	NULL	0	NULL	statement 1	NULL	rate of	is controlled by	NULL				F1	NULL	conformational changes of	IF1 binding site		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_11_9927_s_48	15640141	A model is proposed where the rate of IF1 binding to F1 is controlled by changes in the conformation of the IF1 binding site on F1, which depends on the catalytic state of the enzyme.	bind
42504	3	10998	6	NULL	NULL	0	NULL	F1	NULL	conformational change of	depends on	NULL		IF1 binding site		enzyme	NULL	catalytic state of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_11_9927_s_48	15640141	A model is proposed where the rate of IF1 binding to F1 is controlled by changes in the conformation of the IF1 binding site on F1, which depends on the catalytic state of the enzyme.	bind
50172	1	10999	5	13	NULL	NULL	NULL	RIP140	GP		bind			AF-2		holo-RARholo-RXR	GP		AF-2		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_44_31320_s_246	10531331	A model is proposed wherein RIP140 also binds to holo-RARholo-RXR in a 2:1 ratio through the AF-2 of both receptors (Fig.  7 A).	bind
42272	1	10999	6	NULL	NULL	0	NULL	RIP140	NULL		bind	NULL		AF-2		holo-RARholo-RXR	NULL		AF-2		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_44_31320_s_246	10531331	A model is proposed wherein RIP140 also binds to holo-RARholo-RXR in a 2:1 ratio through the AF-2 of both receptors (Fig.  7 A).	bind
50173	1	11000	5	10	NULL	NULL	NULL	LGL	Cell		bind					target cell	Cell				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-immunol_143_2_2544649_s_12	2544649	A model is proposed,  whereby subsequent to binding of LGL to target cell the large granules  fuse to the LGL plasma membrane and release the small vesicles into the  binding pocket.	bind
50174	2	11000	5	10	NULL	NULL	NULL	large granules	CellComponent		fuse to					LGL plasma membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-immunol_143_2_2544649_s_12	2544649	A model is proposed,  whereby subsequent to binding of LGL to target cell the large granules  fuse to the LGL plasma membrane and release the small vesicles into the  binding pocket.	bind
50175	4	11000	5	10	NULL	NULL	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-immunol_143_2_2544649_s_12	2544649	A model is proposed,  whereby subsequent to binding of LGL to target cell the large granules  fuse to the LGL plasma membrane and release the small vesicles into the  binding pocket.	bind
50176	3	11000	5	10	NULL	NULL	NULL	small vesicles	CellComponent		is released into								binding pocket		NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-immunol_143_2_2544649_s_12	2544649	A model is proposed,  whereby subsequent to binding of LGL to target cell the large granules  fuse to the LGL plasma membrane and release the small vesicles into the  binding pocket.	bind
50177	5	11000	5	10	NULL	NULL	NULL	statement 2	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-immunol_143_2_2544649_s_12	2544649	A model is proposed,  whereby subsequent to binding of LGL to target cell the large granules  fuse to the LGL plasma membrane and release the small vesicles into the  binding pocket.	bind
42505	1	11000	6	10	NULL	NULL	NULL	LGL	Cell		bind					target cell	Cell				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-immunol_143_2_2544649_s_12	2544649	A model is proposed,  whereby subsequent to binding of LGL to target cell the large granules  fuse to the LGL plasma membrane and release the small vesicles into the  binding pocket.	bind
42506	2	11000	6	10	NULL	NULL	NULL	large granules	CellComponent		fuse to					LGL plasma membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-immunol_143_2_2544649_s_12	2544649	A model is proposed,  whereby subsequent to binding of LGL to target cell the large granules  fuse to the LGL plasma membrane and release the small vesicles into the  binding pocket.	bind
42507	3	11000	6	10	NULL	NULL	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-immunol_143_2_2544649_s_12	2544649	A model is proposed,  whereby subsequent to binding of LGL to target cell the large granules  fuse to the LGL plasma membrane and release the small vesicles into the  binding pocket.	bind
42508	4	11000	6	10	NULL	NULL	NULL	small vesicles	CellComponent		released into								binding pocket		NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-immunol_143_2_2544649_s_12	2544649	A model is proposed,  whereby subsequent to binding of LGL to target cell the large granules  fuse to the LGL plasma membrane and release the small vesicles into the  binding pocket.	bind
42509	5	11000	6	10	NULL	NULL	NULL	statement 2	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-immunol_143_2_2544649_s_12	2544649	A model is proposed,  whereby subsequent to binding of LGL to target cell the large granules  fuse to the LGL plasma membrane and release the small vesicles into the  binding pocket.	bind
42510	1	11001	6	10	NULL	NULL	NULL	KAP	GP		interacts with					pCDK2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_615_s_235	11463386	A model of a ternary pCDK2/cyclinA/KAP complex based on our pCDK2/KAPt structure and that of the pCDK2/cyclinA/peptide complex explains these results because it predicts that with the phosphorylated activation segment sequestered at the pCDK2/cyclin A interface, the interaction of KAP with pCDK2 would not interfere with the peptide substrate binding site of CDK2 or the RXL recruitment peptide site of cyclin A   (Figure 5).	bind
42511	2	11001	6	10	NULL	NULL	NULL	statement 1	Process		does not interfere					CDK2	GP		peptide substrate binding site		NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_615_s_235	11463386	A model of a ternary pCDK2/cyclinA/KAP complex based on our pCDK2/KAPt structure and that of the pCDK2/cyclinA/peptide complex explains these results because it predicts that with the phosphorylated activation segment sequestered at the pCDK2/cyclin A interface, the interaction of KAP with pCDK2 would not interfere with the peptide substrate binding site of CDK2 or the RXL recruitment peptide site of cyclin A   (Figure 5).	bind
42512	3	11001	6	10	NULL	NULL	NULL	statement 1	Process		does not interfere with					cyclin A	GP		RXL recruitment peptide site		NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_615_s_235	11463386	A model of a ternary pCDK2/cyclinA/KAP complex based on our pCDK2/KAPt structure and that of the pCDK2/cyclinA/peptide complex explains these results because it predicts that with the phosphorylated activation segment sequestered at the pCDK2/cyclin A interface, the interaction of KAP with pCDK2 would not interfere with the peptide substrate binding site of CDK2 or the RXL recruitment peptide site of cyclin A   (Figure 5).	bind
48987	1	11001	7	10	NULL	NULL	NULL	KAP	GP		interacts with					pCDK2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_615_s_235	11463386	A model of a ternary pCDK2/cyclinA/KAP complex based on our pCDK2/KAPt structure and that of the pCDK2/cyclinA/peptide complex explains these results because it predicts that with the phosphorylated activation segment sequestered at the pCDK2/cyclin A interface, the interaction of KAP with pCDK2 would not interfere with the peptide substrate binding site of CDK2 or the RXL recruitment peptide site of cyclin A   (Figure 5).	bind
48988	2	11001	7	10	NULL	NULL	NULL	statement 1	Process		does not interfere with					CDK2 	GP		peptide substrate binding site 		NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_615_s_235	11463386	A model of a ternary pCDK2/cyclinA/KAP complex based on our pCDK2/KAPt structure and that of the pCDK2/cyclinA/peptide complex explains these results because it predicts that with the phosphorylated activation segment sequestered at the pCDK2/cyclin A interface, the interaction of KAP with pCDK2 would not interfere with the peptide substrate binding site of CDK2 or the RXL recruitment peptide site of cyclin A   (Figure 5).	bind
48989	3	11001	7	10	NULL	NULL	NULL	statement 1	Process		does not interfere with					cyclin A	GP		RXL recruitment peptide site		NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_615_s_235	11463386	A model of a ternary pCDK2/cyclinA/KAP complex based on our pCDK2/KAPt structure and that of the pCDK2/cyclinA/peptide complex explains these results because it predicts that with the phosphorylated activation segment sequestered at the pCDK2/cyclin A interface, the interaction of KAP with pCDK2 would not interfere with the peptide substrate binding site of CDK2 or the RXL recruitment peptide site of cyclin A   (Figure 5).	bind
42273	1	11002	6	10	NULL	NULL	NULL	anthrax toxin lethal factor	GP		bind					protective antigen	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_45_16409_s_1	16251269	A model of anthrax toxin lethal factor bound to protective antigen.	bind
48990	1	11002	7	10	NULL	NULL	NULL	anthrax toxin lethal factor	GP		bind					protective antigen	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_45_16409_s_1	16251269	A model of anthrax toxin lethal factor bound to protective antigen.	bind
42274	1	11004	6	10	NULL	NULL	NULL	apoA-I	GP		bind					ABCA1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_7384_s_309	14660648	A model of apoA-I lipidation  by ABCA1 can be proposed assuming that 1) initial binding of apoA-I to ABCA1 is irreversible  or slowly reversible ( k1"`  k -  1); 2) lipidated apoA-I (alpha-LpA-I-like particles) dissociate rapidly ( k2) from ABCA1 without any detectable reassociation; and 3) this system contains no  other apolipoprotein that could compete for the binding of lipid-free apoA-I to ABCA1.	bind
42513	2	11004	6	10	NULL	NULL	NULL	apo A-I	GP	lipid-free	bind					ABCA1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_7384_s_309	14660648	A model of apoA-I lipidation  by ABCA1 can be proposed assuming that 1) initial binding of apoA-I to ABCA1 is irreversible  or slowly reversible ( k1"`  k -  1); 2) lipidated apoA-I (alpha-LpA-I-like particles) dissociate rapidly ( k2) from ABCA1 without any detectable reassociation; and 3) this system contains no  other apolipoprotein that could compete for the binding of lipid-free apoA-I to ABCA1.	bind
42514	3	11004	6	10	NULL	NULL	NULL	lipidated apoA-I	GP		is					alpha-LpA-I-like particles	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_7384_s_309	14660648	A model of apoA-I lipidation  by ABCA1 can be proposed assuming that 1) initial binding of apoA-I to ABCA1 is irreversible  or slowly reversible ( k1"`  k -  1); 2) lipidated apoA-I (alpha-LpA-I-like particles) dissociate rapidly ( k2) from ABCA1 without any detectable reassociation; and 3) this system contains no  other apolipoprotein that could compete for the binding of lipid-free apoA-I to ABCA1.	bind
42515	4	11004	6	10	NULL	NULL	NULL	apoA-I	GP	lipidated	dissociates from		rapidly			ABCA1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_7384_s_309	14660648	A model of apoA-I lipidation  by ABCA1 can be proposed assuming that 1) initial binding of apoA-I to ABCA1 is irreversible  or slowly reversible ( k1"`  k -  1); 2) lipidated apoA-I (alpha-LpA-I-like particles) dissociate rapidly ( k2) from ABCA1 without any detectable reassociation; and 3) this system contains no  other apolipoprotein that could compete for the binding of lipid-free apoA-I to ABCA1.	bind
48991	1	11004	7	10	NULL	NULL	NULL	apoA-I	GP		bind					ABCA1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_7384_s_309	14660648	A model of apoA-I lipidation  by ABCA1 can be proposed assuming that 1) initial binding of apoA-I to ABCA1 is irreversible  or slowly reversible ( k1"`  k -  1); 2) lipidated apoA-I (alpha-LpA-I-like particles) dissociate rapidly ( k2) from ABCA1 without any detectable reassociation; and 3) this system contains no  other apolipoprotein that could compete for the binding of lipid-free apoA-I to ABCA1.	bind
48992	2	11004	7	10	NULL	NULL	NULL	statement 1	Process		is a type of					irreversible reaction	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_7384_s_309	14660648	A model of apoA-I lipidation  by ABCA1 can be proposed assuming that 1) initial binding of apoA-I to ABCA1 is irreversible  or slowly reversible ( k1"`  k -  1); 2) lipidated apoA-I (alpha-LpA-I-like particles) dissociate rapidly ( k2) from ABCA1 without any detectable reassociation; and 3) this system contains no  other apolipoprotein that could compete for the binding of lipid-free apoA-I to ABCA1.	bind
48993	3	11004	7	10	NULL	NULL	NULL	statement 1	Process		is a type of					slowly reversible reaction	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_7384_s_309	14660648	A model of apoA-I lipidation  by ABCA1 can be proposed assuming that 1) initial binding of apoA-I to ABCA1 is irreversible  or slowly reversible ( k1"`  k -  1); 2) lipidated apoA-I (alpha-LpA-I-like particles) dissociate rapidly ( k2) from ABCA1 without any detectable reassociation; and 3) this system contains no  other apolipoprotein that could compete for the binding of lipid-free apoA-I to ABCA1.	bind
48994	4	11004	7	10	NULL	NULL	NULL	 apoA-I	GP	lipidated	dissociate from		rapidly			ABCA1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_7384_s_309	14660648	A model of apoA-I lipidation  by ABCA1 can be proposed assuming that 1) initial binding of apoA-I to ABCA1 is irreversible  or slowly reversible ( k1"`  k -  1); 2) lipidated apoA-I (alpha-LpA-I-like particles) dissociate rapidly ( k2) from ABCA1 without any detectable reassociation; and 3) this system contains no  other apolipoprotein that could compete for the binding of lipid-free apoA-I to ABCA1.	bind
48995	5	11004	7	10	NULL	NULL	NULL	apoA-I 	GP	lipid-free 	bind					ABCA1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_7384_s_309	14660648	A model of apoA-I lipidation  by ABCA1 can be proposed assuming that 1) initial binding of apoA-I to ABCA1 is irreversible  or slowly reversible ( k1"`  k -  1); 2) lipidated apoA-I (alpha-LpA-I-like particles) dissociate rapidly ( k2) from ABCA1 without any detectable reassociation; and 3) this system contains no  other apolipoprotein that could compete for the binding of lipid-free apoA-I to ABCA1.	bind
48996	6	11004	7	10	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_7384_s_309	14660648	A model of apoA-I lipidation  by ABCA1 can be proposed assuming that 1) initial binding of apoA-I to ABCA1 is irreversible  or slowly reversible ( k1"`  k -  1); 2) lipidated apoA-I (alpha-LpA-I-like particles) dissociate rapidly ( k2) from ABCA1 without any detectable reassociation; and 3) this system contains no  other apolipoprotein that could compete for the binding of lipid-free apoA-I to ABCA1.	bind
49037	7	11004	7	10	NULL	NULL	NULL	statement 4	Process		does not					reassociate	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_7384_s_309	14660648	A model of apoA-I lipidation  by ABCA1 can be proposed assuming that 1) initial binding of apoA-I to ABCA1 is irreversible  or slowly reversible ( k1"`  k -  1); 2) lipidated apoA-I (alpha-LpA-I-like particles) dissociate rapidly ( k2) from ABCA1 without any detectable reassociation; and 3) this system contains no  other apolipoprotein that could compete for the binding of lipid-free apoA-I to ABCA1.	bind
49039	8	11004	7	10	NULL	NULL	NULL	lipidated apoA-I	GP		is					alpha-LpA-I-like particles	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_7384_s_309	14660648	A model of apoA-I lipidation  by ABCA1 can be proposed assuming that 1) initial binding of apoA-I to ABCA1 is irreversible  or slowly reversible ( k1"`  k -  1); 2) lipidated apoA-I (alpha-LpA-I-like particles) dissociate rapidly ( k2) from ABCA1 without any detectable reassociation; and 3) this system contains no  other apolipoprotein that could compete for the binding of lipid-free apoA-I to ABCA1.	bind
42275	1	11005	6	10	NULL	NULL	NULL	Cry1Ac	GP		bind		bivalent;;sequentially			APN	GP	L. dispar			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_19_14423_s_291	10799525	A model of bivalent sequential binding of Cry1Ac to  L. dispar APN.	bind
49040	1	11005	7	10	NULL	NULL	NULL	Cry1Ac	GP		bind		bivalent;;sequentially			APN	GP	L. dispar 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_19_14423_s_291	10799525	A model of bivalent sequential binding of Cry1Ac to  L. dispar APN.	bind
42276	1	11006	6	10	NULL	NULL	NULL	calmodulin	GP	Ca(2+)-free	bind					myosin	GP	unconventional			NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_structure_4_12_8994973_s_1	8994973	A model of Ca(2+)-free calmodulin binding to unconventional myosins reveals how calmodulin acts as a regulatory switch..	bind
42278	2	11006	6	10	NULL	NULL	NULL	calmodulin	GP		acts as a					regulatory switch	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_structure_4_12_8994973_s_1	8994973	A model of Ca(2+)-free calmodulin binding to unconventional myosins reveals how calmodulin acts as a regulatory switch..	bind
42279	3	11006	6	10	NULL	NULL	NULL	statement 1	Process		reveals					statement 2	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_structure_4_12_8994973_s_1	8994973	A model of Ca(2+)-free calmodulin binding to unconventional myosins reveals how calmodulin acts as a regulatory switch..	bind
49041	1	11006	7	10	NULL	NULL	NULL	calmodulin 	GP	Ca(2+)-free	bind					myosins	GP	unconventional			NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_structure_4_12_8994973_s_1	8994973	A model of Ca(2+)-free calmodulin binding to unconventional myosins reveals how calmodulin acts as a regulatory switch..	bind
49042	2	11006	7	10	NULL	NULL	NULL	calmodulin	GP		acts as a 					regular switch	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_structure_4_12_8994973_s_1	8994973	A model of Ca(2+)-free calmodulin binding to unconventional myosins reveals how calmodulin acts as a regulatory switch..	bind
49043	3	11006	7	10	NULL	NULL	NULL	statement 1	Process		reveals					statement 2	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_structure_4_12_8994973_s_1	8994973	A model of Ca(2+)-free calmodulin binding to unconventional myosins reveals how calmodulin acts as a regulatory switch..	bind
42280	1	11009	6	10	NULL	NULL	NULL	calmodulin	GP		bind								IQ motif		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_6_4347_s_192	12446675	A model of calmodulin bound to an IQ motif has been constructed, using the crystal structure of the regulatory domain of scallop myosin ( ,  ).	bind
49050	1	11009	7	10	NULL	NULL	NULL	calmodulin	GP		bind								IQ motif		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_6_4347_s_192	12446675	A model of calmodulin bound to an IQ motif has been constructed, using the crystal structure of the regulatory domain of scallop myosin ( ,  ).	bind
42281	1	11011	6	10	NULL	NULL	NULL	cGMP	Chemical		bind					delta1-52PKG-Ibeta	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_5_2380_s_5	12591946	A model of cGMP binding to delta1-52PKG-Ibeta indicates that elongation of delta1-52PKG-Ibeta requires binding of cGMP to the low-affinity binding site of the R domain.	bind
42282	2	11011	6	10	NULL	NULL	NULL	cGMP	Chemical		bind							low affinity	binding site of the R domain		NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_5_2380_s_5	12591946	A model of cGMP binding to delta1-52PKG-Ibeta indicates that elongation of delta1-52PKG-Ibeta requires binding of cGMP to the low-affinity binding site of the R domain.	bind
42283	3	11011	6	10	NULL	NULL	NULL	statement 2	Process		is required for					delta1-52PKG-Ibeta	GP	elongation of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_5_2380_s_5	12591946	A model of cGMP binding to delta1-52PKG-Ibeta indicates that elongation of delta1-52PKG-Ibeta requires binding of cGMP to the low-affinity binding site of the R domain.	bind
49051	1	11011	7	10	NULL	NULL	NULL	cGMP 	Chemical		bind					delta1-52PKG-Ibeta	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_5_2380_s_5	12591946	A model of cGMP binding to delta1-52PKG-Ibeta indicates that elongation of delta1-52PKG-Ibeta requires binding of cGMP to the low-affinity binding site of the R domain.	bind
49053	2	11011	7	10	NULL	NULL	NULL	 cGMP	Chemical		bind							low-affinity	binding site of R domain		NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_5_2380_s_5	12591946	A model of cGMP binding to delta1-52PKG-Ibeta indicates that elongation of delta1-52PKG-Ibeta requires binding of cGMP to the low-affinity binding site of the R domain.	bind
49054	3	11011	7	10	NULL	NULL	NULL	delta1-52PKG-Ibeta	GP	elongation of	requires					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_100_5_2380_s_5	12591946	A model of cGMP binding to delta1-52PKG-Ibeta indicates that elongation of delta1-52PKG-Ibeta requires binding of cGMP to the low-affinity binding site of the R domain.	bind
42284	1	11012	6	10	NULL	NULL	NULL	dimeric ligand	GP		bind					monomeric receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_14_2_135_s_170	11239446	A Model of Dimeric Ligand Binding to Monomeric Receptors	bind
49055	1	11012	7	10	NULL	NULL	NULL	Dimeric Ligand 	GP		bind					monomeric receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_14_2_135_s_170	11239446	A Model of Dimeric Ligand Binding to Monomeric Receptors	bind
42285	1	11014	6	10	NULL	NULL	NULL	glutamine	AminoAcid		bind					GlnRS	GP				NULL		NULL	NULL	NULL	NULL	gw60_structure_6_4_439_s_35	9562563	A model of glutamine bound to GlnRS was proposed based on the observed positions of ATP and adenine 76 (A76) of the tRNA  [6  .	bind
49056	1	11014	7	10	NULL	NULL	NULL	glutamine 	AminoAcid		bind					GlnRS	GP				NULL		NULL	NULL	NULL	NULL	gw60_structure_6_4_439_s_35	9562563	A model of glutamine bound to GlnRS was proposed based on the observed positions of ATP and adenine 76 (A76) of the tRNA  [6  .	bind
42287	2	11015	6	10	NULL	NULL	NULL	mAb 2G12 Fab2	GP		bind					HIV-1 Env spike					NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_42_14943_s_125	16219699	A model of mAb 2G12 Fab2 bound to the HIV-1 Env spike.	bind
49060	1	11015	7	10	NULL	NULL	NULL	mAb 2G12 Fab2	GP		bind					HIV-1 Env spike					NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_42_14943_s_125	16219699	A model of mAb 2G12 Fab2 bound to the HIV-1 Env spike.	bind
42288	1	11016	6	10	NULL	NULL	NULL	tRNA	NucleicAcid	bipartite precursor	bind					hLa protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_2_367_s_245	11134326	A model of phosphorylation-regulated, bipartite precursor tRNA binding by the hLa protein.	bind
42289	2	11016	6	10	NULL	NULL	NULL	statement 1	Process		is regulated by					phosphorylation	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_2_367_s_245	11134326	A model of phosphorylation-regulated, bipartite precursor tRNA binding by the hLa protein.	bind
49063	1	11016	7	10	NULL	NULL	NULL	hLa protein	GP		bind					tRNA	NucleicAcid	bipartite precursor			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_2_367_s_245	11134326	A model of phosphorylation-regulated, bipartite precursor tRNA binding by the hLa protein.	bind
49064	2	11016	7	10	NULL	NULL	NULL	phosphorylation	Process		regulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_2_367_s_245	11134326	A model of phosphorylation-regulated, bipartite precursor tRNA binding by the hLa protein.	bind
42516	1	11017	6	10	NULL	NULL	NULL	Immunophilin	GP		bind			tetratricopeptide repeat domain		hsp90	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_32_18841_s_244	7642537	A Model of Protein Targeting Mediated by Immunophilins and Other Proteins That Bind to hsp90 via Tetratricopeptide Repeat Domains.	bind
49065	1	11017	7	10	NULL	NULL	NULL	Immunophilins	GP		bind			Tetratricopeptide Repeat Domains		hsp90	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_32_18841_s_244	7642537	A Model of Protein Targeting Mediated by Immunophilins and Other Proteins That Bind to hsp90 via Tetratricopeptide Repeat Domains.	bind
42517	1	11018	6	10	NULL	NULL	NULL	GTP	Chemical		bind					Galpha subunit	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_13_11115_s_336	12538649	A model of RGS4 regulation by the anionic phospholipid  PA. Agonist-induced stimulation of G-protein-coupled receptors enhances GTP binding  to Galpha subunits.	bind
42518	2	11018	6	10	NULL	NULL	NULL	PA	Chemical		is a type of					anionic phospholipid	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_13_11115_s_336	12538649	A model of RGS4 regulation by the anionic phospholipid  PA. Agonist-induced stimulation of G-protein-coupled receptors enhances GTP binding  to Galpha subunits.	bind
42519	3	11018	6	10	NULL	NULL	NULL	PA	Chemical		regulates					RGS4	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_13_11115_s_336	12538649	A model of RGS4 regulation by the anionic phospholipid  PA. Agonist-induced stimulation of G-protein-coupled receptors enhances GTP binding  to Galpha subunits.	bind
42520	4	11018	6	10	NULL	NULL	NULL	agonist	Chemical		induces					G-protein-coupled receptors 	GP	stimulation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_13_11115_s_336	12538649	A model of RGS4 regulation by the anionic phospholipid  PA. Agonist-induced stimulation of G-protein-coupled receptors enhances GTP binding  to Galpha subunits.	bind
42521	5	11018	6	10	NULL	NULL	NULL	statement 4	Process		enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_13_11115_s_336	12538649	A model of RGS4 regulation by the anionic phospholipid  PA. Agonist-induced stimulation of G-protein-coupled receptors enhances GTP binding  to Galpha subunits.	bind
49066	1	11018	7	10	NULL	NULL	NULL	PA	Chemical		regulates					RGS4	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_13_11115_s_336	12538649	A model of RGS4 regulation by the anionic phospholipid  PA. Agonist-induced stimulation of G-protein-coupled receptors enhances GTP binding  to Galpha subunits.	bind
49067	2	11018	7	10	NULL	NULL	NULL	GTP	Chemical		bind					Galpha subunits	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_13_11115_s_336	12538649	A model of RGS4 regulation by the anionic phospholipid  PA. Agonist-induced stimulation of G-protein-coupled receptors enhances GTP binding  to Galpha subunits.	bind
49068	3	11018	7	10	NULL	NULL	NULL	Agonist	Chemical		induce					G-protein-coupled receptors	GP	stimulation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_13_11115_s_336	12538649	A model of RGS4 regulation by the anionic phospholipid  PA. Agonist-induced stimulation of G-protein-coupled receptors enhances GTP binding  to Galpha subunits.	bind
49069	4	11018	7	10	NULL	NULL	NULL	statement 3	Process		enhance					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_13_11115_s_336	12538649	A model of RGS4 regulation by the anionic phospholipid  PA. Agonist-induced stimulation of G-protein-coupled receptors enhances GTP binding  to Galpha subunits.	bind
50266	5	11018	7	10	NULL	NULL	NULL	PA	Chemical		is a type of					anionic phospholipid	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_13_11115_s_336	12538649	A model of RGS4 regulation by the anionic phospholipid  PA. Agonist-induced stimulation of G-protein-coupled receptors enhances GTP binding  to Galpha subunits.	bind
42294	1	11020	6	10	NULL	NULL	NULL	SecA	GP		bind					SecB	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_mol-microbiol_58_2_16194224_s_8	16194224	A model of SecB-SecA complex suggests that  the binding of SecA to SecB changes the conformation of the polypeptide  binding sites in the chaperone, enabling transfer of precursor polypeptides  from SecB to SecA.	bind
42297	2	11020	6	10	NULL	NULL	NULL	statement 1	Process		changes					chaperone	GP	conformation of	polypeptide binding site		NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_mol-microbiol_58_2_16194224_s_8	16194224	A model of SecB-SecA complex suggests that  the binding of SecA to SecB changes the conformation of the polypeptide  binding sites in the chaperone, enabling transfer of precursor polypeptides  from SecB to SecA.	bind
42298	3	11020	6	10	NULL	NULL	NULL	precursor polypeptides	AminoAcid		are transfered to					SecA	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_mol-microbiol_58_2_16194224_s_8	16194224	A model of SecB-SecA complex suggests that  the binding of SecA to SecB changes the conformation of the polypeptide  binding sites in the chaperone, enabling transfer of precursor polypeptides  from SecB to SecA.	bind
42300	4	11020	6	10	NULL	NULL	NULL	statement 2	Process		enables					statement 3	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_mol-microbiol_58_2_16194224_s_8	16194224	A model of SecB-SecA complex suggests that  the binding of SecA to SecB changes the conformation of the polypeptide  binding sites in the chaperone, enabling transfer of precursor polypeptides  from SecB to SecA.	bind
50267	5	11020	6	10	NULL	NULL	NULL	precursor polypeptides \t	AminoAcid		is transfered from					SecB	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_mol-microbiol_58_2_16194224_s_8	16194224	A model of SecB-SecA complex suggests that  the binding of SecA to SecB changes the conformation of the polypeptide  binding sites in the chaperone, enabling transfer of precursor polypeptides  from SecB to SecA.	bind
50268	6	11020	6	10	NULL	NULL	NULL	statement 5	Process		occurs simultaneously with					statement 3	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_mol-microbiol_58_2_16194224_s_8	16194224	A model of SecB-SecA complex suggests that  the binding of SecA to SecB changes the conformation of the polypeptide  binding sites in the chaperone, enabling transfer of precursor polypeptides  from SecB to SecA.	bind
49070	1	11020	7	10	NULL	NULL	NULL	SecA 	GP		bind					SecB	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_mol-microbiol_58_2_16194224_s_8	16194224	A model of SecB-SecA complex suggests that  the binding of SecA to SecB changes the conformation of the polypeptide  binding sites in the chaperone, enabling transfer of precursor polypeptides  from SecB to SecA.	bind
49071	2	11020	7	10	NULL	NULL	NULL	statement 1	Process		changes					chaperone	GP	conformation of	polypeptide binding sites		NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_mol-microbiol_58_2_16194224_s_8	16194224	A model of SecB-SecA complex suggests that  the binding of SecA to SecB changes the conformation of the polypeptide  binding sites in the chaperone, enabling transfer of precursor polypeptides  from SecB to SecA.	bind
49072	3	11020	7	10	NULL	NULL	NULL	precursor polypeptide	AminoAcid		transferred from					SecB	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_mol-microbiol_58_2_16194224_s_8	16194224	A model of SecB-SecA complex suggests that  the binding of SecA to SecB changes the conformation of the polypeptide  binding sites in the chaperone, enabling transfer of precursor polypeptides  from SecB to SecA.	bind
49073	4	11020	7	10	NULL	NULL	NULL	precursor polypeptide	AminoAcid		transferred to					SecA	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_mol-microbiol_58_2_16194224_s_8	16194224	A model of SecB-SecA complex suggests that  the binding of SecA to SecB changes the conformation of the polypeptide  binding sites in the chaperone, enabling transfer of precursor polypeptides  from SecB to SecA.	bind
49074	5	11020	7	10	NULL	NULL	NULL	statement 3	Process		occur simultaneously with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_mol-microbiol_58_2_16194224_s_8	16194224	A model of SecB-SecA complex suggests that  the binding of SecA to SecB changes the conformation of the polypeptide  binding sites in the chaperone, enabling transfer of precursor polypeptides  from SecB to SecA.	bind
49075	6	11020	7	10	NULL	NULL	NULL	statement 2	Process		enables					statement 5	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_mol-microbiol_58_2_16194224_s_8	16194224	A model of SecB-SecA complex suggests that  the binding of SecA to SecB changes the conformation of the polypeptide  binding sites in the chaperone, enabling transfer of precursor polypeptides  from SecB to SecA.	bind
42522	1	11021	6	10	NULL	NULL	NULL	DAG	Chemical		bind					UNC-13	GP				NULL	C. elegans	NULL	NULL	NULL	NULL	gw70_genetics_169_2_651_s_235	15489511	A model of the  C. elegans EGL-30 (Galphaq) pathway predicts that this is caused by increased synaptic vesicle priming, in part via DAG-mediated activation of the UNC-13 synaptic vesicle priming protein ( Figure 1A); however, a prior study suggests that UNC-13-mediated synaptic vesicle priming is not dependent on DAG binding to UNC-13, because eliminating the ability of UNC-13 to bind DAG does not significantly affect neurotransmitter release ( HEE et al.).	bind
42523	2	11021	6	10	NULL	NULL	NULL	statement 1	Process	elimination of	does not affect		significantly			neurotransmitter	Process	release of			NULL	C. elegans	NULL	NULL	NULL	NULL	gw70_genetics_169_2_651_s_235	15489511	A model of the  C. elegans EGL-30 (Galphaq) pathway predicts that this is caused by increased synaptic vesicle priming, in part via DAG-mediated activation of the UNC-13 synaptic vesicle priming protein ( Figure 1A); however, a prior study suggests that UNC-13-mediated synaptic vesicle priming is not dependent on DAG binding to UNC-13, because eliminating the ability of UNC-13 to bind DAG does not significantly affect neurotransmitter release ( HEE et al.).	bind
42540	3	11021	6	10	NULL	NULL	NULL	UNC-13	GP		mediates					synaptic vesicle	CellComponent	priming of 			NULL	C. elegans	NULL	NULL	NULL	NULL	gw70_genetics_169_2_651_s_235	15489511	A model of the  C. elegans EGL-30 (Galphaq) pathway predicts that this is caused by increased synaptic vesicle priming, in part via DAG-mediated activation of the UNC-13 synaptic vesicle priming protein ( Figure 1A); however, a prior study suggests that UNC-13-mediated synaptic vesicle priming is not dependent on DAG binding to UNC-13, because eliminating the ability of UNC-13 to bind DAG does not significantly affect neurotransmitter release ( HEE et al.).	bind
42541	4	11021	6	10	NULL	NULL	NULL	statement 1	Process		is independent of					statement 3	Process				NULL	C. elegans	NULL	NULL	NULL	NULL	gw70_genetics_169_2_651_s_235	15489511	A model of the  C. elegans EGL-30 (Galphaq) pathway predicts that this is caused by increased synaptic vesicle priming, in part via DAG-mediated activation of the UNC-13 synaptic vesicle priming protein ( Figure 1A); however, a prior study suggests that UNC-13-mediated synaptic vesicle priming is not dependent on DAG binding to UNC-13, because eliminating the ability of UNC-13 to bind DAG does not significantly affect neurotransmitter release ( HEE et al.).	bind
50269	5	11021	6	10	NULL	NULL	NULL	DAG	Chemical		mediate					UNC-13 synaptic vesicle priming protein 	GP	activation of			NULL	C. elegans	NULL	NULL	NULL	NULL	gw70_genetics_169_2_651_s_235	15489511	A model of the  C. elegans EGL-30 (Galphaq) pathway predicts that this is caused by increased synaptic vesicle priming, in part via DAG-mediated activation of the UNC-13 synaptic vesicle priming protein ( Figure 1A); however, a prior study suggests that UNC-13-mediated synaptic vesicle priming is not dependent on DAG binding to UNC-13, because eliminating the ability of UNC-13 to bind DAG does not significantly affect neurotransmitter release ( HEE et al.).	bind
49076	1	11021	7	10	NULL	NULL	NULL	DAG	Chemical		mediates					UNC-13 synaptic vesicle priming protein 	GP	activation of			NULL	C.elegans	NULL	NULL	NULL	NULL	gw70_genetics_169_2_651_s_235	15489511	A model of the  C. elegans EGL-30 (Galphaq) pathway predicts that this is caused by increased synaptic vesicle priming, in part via DAG-mediated activation of the UNC-13 synaptic vesicle priming protein ( Figure 1A); however, a prior study suggests that UNC-13-mediated synaptic vesicle priming is not dependent on DAG binding to UNC-13, because eliminating the ability of UNC-13 to bind DAG does not significantly affect neurotransmitter release ( HEE et al.).	bind
49078	3	11021	7	10	NULL	NULL	NULL	 DAG	Chemical		bind					UNC-13	GP				NULL	C.elegans	NULL	NULL	NULL	NULL	gw70_genetics_169_2_651_s_235	15489511	A model of the  C. elegans EGL-30 (Galphaq) pathway predicts that this is caused by increased synaptic vesicle priming, in part via DAG-mediated activation of the UNC-13 synaptic vesicle priming protein ( Figure 1A); however, a prior study suggests that UNC-13-mediated synaptic vesicle priming is not dependent on DAG binding to UNC-13, because eliminating the ability of UNC-13 to bind DAG does not significantly affect neurotransmitter release ( HEE et al.).	bind
49079	4	11021	7	10	NULL	NULL	NULL	UNC-13	GP		mediates					synaptic vesicle 	CellComponent	priming of			NULL	C.elegans	NULL	NULL	NULL	NULL	gw70_genetics_169_2_651_s_235	15489511	A model of the  C. elegans EGL-30 (Galphaq) pathway predicts that this is caused by increased synaptic vesicle priming, in part via DAG-mediated activation of the UNC-13 synaptic vesicle priming protein ( Figure 1A); however, a prior study suggests that UNC-13-mediated synaptic vesicle priming is not dependent on DAG binding to UNC-13, because eliminating the ability of UNC-13 to bind DAG does not significantly affect neurotransmitter release ( HEE et al.).	bind
49080	5	11021	7	10	NULL	NULL	NULL	statement 4	Process		does not depend on					statement 3	Process				NULL	C.elegans	NULL	NULL	NULL	NULL	gw70_genetics_169_2_651_s_235	15489511	A model of the  C. elegans EGL-30 (Galphaq) pathway predicts that this is caused by increased synaptic vesicle priming, in part via DAG-mediated activation of the UNC-13 synaptic vesicle priming protein ( Figure 1A); however, a prior study suggests that UNC-13-mediated synaptic vesicle priming is not dependent on DAG binding to UNC-13, because eliminating the ability of UNC-13 to bind DAG does not significantly affect neurotransmitter release ( HEE et al.).	bind
49081	6	11021	7	10	NULL	NULL	NULL	statement 3	Process	elimination of	does not affect					neurotransmitter	Chemical	release of			NULL	C.elegans	NULL	NULL	NULL	NULL	gw70_genetics_169_2_651_s_235	15489511	A model of the  C. elegans EGL-30 (Galphaq) pathway predicts that this is caused by increased synaptic vesicle priming, in part via DAG-mediated activation of the UNC-13 synaptic vesicle priming protein ( Figure 1A); however, a prior study suggests that UNC-13-mediated synaptic vesicle priming is not dependent on DAG binding to UNC-13, because eliminating the ability of UNC-13 to bind DAG does not significantly affect neurotransmitter release ( HEE et al.).	bind
42301	1	11022	6	10	NULL	NULL	NULL	AC1	GP		bind			C1 domain		Gsalpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_25_13414_s_36	9391039	A model of the AC1 C1/AC2 C2 heterodimer was used to predict a region on the AC1 C1 domain that binds Gsalpha ( 20).	bind
49082	1	11022	7	10	NULL	NULL	NULL	AC1	GP		bind			C1 domain		Gsalpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_25_13414_s_36	9391039	A model of the AC1 C1/AC2 C2 heterodimer was used to predict a region on the AC1 C1 domain that binds Gsalpha ( 20).	bind
42567	1	11023	6	10	NULL	NULL	NULL	CipA	GP		bind			type II dockerin		SdbA 	GP		cohesin domain		NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_1_124_s_378	15755956	A model of the attachment of CipA to the cell involving use of its type II dockerin binding to a cohesin domain in the SdbA cell surface protein was proposed by Beguin and Alzari ( ).	bind
42568	2	11023	6	10	NULL	NULL	NULL	SdbA	GP		is a type of					cell surface protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_1_124_s_378	15755956	A model of the attachment of CipA to the cell involving use of its type II dockerin binding to a cohesin domain in the SdbA cell surface protein was proposed by Beguin and Alzari ( ).	bind
49083	1	11023	7	10	NULL	NULL	NULL	CipA	GP		bind			type II dockerin		SdbA	GP		cohesin domain		NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_1_124_s_378	15755956	A model of the attachment of CipA to the cell involving use of its type II dockerin binding to a cohesin domain in the SdbA cell surface protein was proposed by Beguin and Alzari ( ).	bind
49084	2	11023	7	10	NULL	NULL	NULL	SdbA	GP		is a type of					cell surface protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_1_124_s_378	15755956	A model of the attachment of CipA to the cell involving use of its type II dockerin binding to a cohesin domain in the SdbA cell surface protein was proposed by Beguin and Alzari ( ).	bind
42302	1	11024	6	10	NULL	NULL	NULL	Galphai1	GP		bind			helical domain		RGS14	GP		GL		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_45_46772_s_171	15337739	A model of the Galphai1 helical domain that binds to RGS14-GL is shown in  Fig. 5 A.	bind
49085	1	11024	7	10	NULL	NULL	NULL	Galphai1	GP		bind			helical domain 		RGS14	GP		GL		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_45_46772_s_171	15337739	A model of the Galphai1 helical domain that binds to RGS14-GL is shown in  Fig. 5 A.	bind
42303	1	11025	6	10	NULL	NULL	NULL	tyrphostin A25	Chemical		bind					CyaC	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_31754_s_162	16002394	A model of the most effective tyrphostin A25 bound to CyaC may be generated without creating steric clash by superposition of the tyrphostin on the CE of the CyaC.2-CE complex ( Fig. 4 C).	bind
49086	1	11025	7	10	NULL	NULL	NULL	tyrphostin A25	Chemical		bind					CyaC	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_36_31754_s_162	16002394	A model of the most effective tyrphostin A25 bound to CyaC may be generated without creating steric clash by superposition of the tyrphostin on the CE of the CyaC.2-CE complex ( Fig. 4 C).	bind
42304	1	11027	6	10	NULL	NULL	NULL	Rad9	GP		bind					FHA2	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5374_185_s_43	9687277	A model presents itself: Rad9 binds to FHA2 to mediate the Rad53 response during G1 or G2 while another protein, perhaps polymerase e, binds to FHA1 to mediate the Rad53 response during S phase (see the figure).	bind
42331	2	11027	6	10	NULL	NULL	NULL	polymerase e	GP		bind		may			FHA1	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5374_185_s_43	9687277	A model presents itself: Rad9 binds to FHA2 to mediate the Rad53 response during G1 or G2 while another protein, perhaps polymerase e, binds to FHA1 to mediate the Rad53 response during S phase (see the figure).	bind
42332	3	11027	6	10	NULL	NULL	NULL	statement 1	Process		mediates					Rad53	GP	response of 			NULL		NULL	NULL	NULL	NULL	gw60_science_281_5374_185_s_43	9687277	A model presents itself: Rad9 binds to FHA2 to mediate the Rad53 response during G1 or G2 while another protein, perhaps polymerase e, binds to FHA1 to mediate the Rad53 response during S phase (see the figure).	bind
42333	4	11027	6	10	NULL	NULL	NULL	statement 3	Process		occurs during					G1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5374_185_s_43	9687277	A model presents itself: Rad9 binds to FHA2 to mediate the Rad53 response during G1 or G2 while another protein, perhaps polymerase e, binds to FHA1 to mediate the Rad53 response during S phase (see the figure).	bind
42334	5	11027	6	10	NULL	NULL	NULL	statement 3	Process		occurs during					G2	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5374_185_s_43	9687277	A model presents itself: Rad9 binds to FHA2 to mediate the Rad53 response during G1 or G2 while another protein, perhaps polymerase e, binds to FHA1 to mediate the Rad53 response during S phase (see the figure).	bind
42336	6	11027	6	10	NULL	NULL	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5374_185_s_43	9687277	A model presents itself: Rad9 binds to FHA2 to mediate the Rad53 response during G1 or G2 while another protein, perhaps polymerase e, binds to FHA1 to mediate the Rad53 response during S phase (see the figure).	bind
42343	7	11027	6	10	NULL	NULL	NULL	statement 2	Process		mediates					Rad53	GP	response of			NULL		NULL	NULL	NULL	NULL	gw60_science_281_5374_185_s_43	9687277	A model presents itself: Rad9 binds to FHA2 to mediate the Rad53 response during G1 or G2 while another protein, perhaps polymerase e, binds to FHA1 to mediate the Rad53 response during S phase (see the figure).	bind
42345	8	11027	6	10	NULL	NULL	NULL	statement 7	Process		occurs during					S phase	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5374_185_s_43	9687277	A model presents itself: Rad9 binds to FHA2 to mediate the Rad53 response during G1 or G2 while another protein, perhaps polymerase e, binds to FHA1 to mediate the Rad53 response during S phase (see the figure).	bind
49087	1	11027	7	10	NULL	NULL	NULL	Rad9 	GP		bind					FHA2	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5374_185_s_43	9687277	A model presents itself: Rad9 binds to FHA2 to mediate the Rad53 response during G1 or G2 while another protein, perhaps polymerase e, binds to FHA1 to mediate the Rad53 response during S phase (see the figure).	bind
49088	2	11027	7	10	NULL	NULL	NULL	statement 1	Process		mediate					Rad53	GP	response of			NULL		NULL	NULL	NULL	NULL	gw60_science_281_5374_185_s_43	9687277	A model presents itself: Rad9 binds to FHA2 to mediate the Rad53 response during G1 or G2 while another protein, perhaps polymerase e, binds to FHA1 to mediate the Rad53 response during S phase (see the figure).	bind
49089	3	11027	7	10	NULL	NULL	NULL	statement 2	Process		occur during					G1 phase	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5374_185_s_43	9687277	A model presents itself: Rad9 binds to FHA2 to mediate the Rad53 response during G1 or G2 while another protein, perhaps polymerase e, binds to FHA1 to mediate the Rad53 response during S phase (see the figure).	bind
49090	4	11027	7	10	NULL	NULL	NULL	statement 2	Process		occur during					G2 phase	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5374_185_s_43	9687277	A model presents itself: Rad9 binds to FHA2 to mediate the Rad53 response during G1 or G2 while another protein, perhaps polymerase e, binds to FHA1 to mediate the Rad53 response during S phase (see the figure).	bind
49091	5	11027	7	10	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5374_185_s_43	9687277	A model presents itself: Rad9 binds to FHA2 to mediate the Rad53 response during G1 or G2 while another protein, perhaps polymerase e, binds to FHA1 to mediate the Rad53 response during S phase (see the figure).	bind
49092	6	11027	7	10	NULL	NULL	NULL	polymerase e	GP		bind					FHA1	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5374_185_s_43	9687277	A model presents itself: Rad9 binds to FHA2 to mediate the Rad53 response during G1 or G2 while another protein, perhaps polymerase e, binds to FHA1 to mediate the Rad53 response during S phase (see the figure).	bind
49093	7	11027	7	10	NULL	NULL	NULL	statement 6	Process		mediate					Rad53	GP	response of			NULL		NULL	NULL	NULL	NULL	gw60_science_281_5374_185_s_43	9687277	A model presents itself: Rad9 binds to FHA2 to mediate the Rad53 response during G1 or G2 while another protein, perhaps polymerase e, binds to FHA1 to mediate the Rad53 response during S phase (see the figure).	bind
49094	8	11027	7	10	NULL	NULL	NULL	statement 7	Process		occur during					S phase	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5374_185_s_43	9687277	A model presents itself: Rad9 binds to FHA2 to mediate the Rad53 response during G1 or G2 while another protein, perhaps polymerase e, binds to FHA1 to mediate the Rad53 response during S phase (see the figure).	bind
42542	1	11028	6	10	NULL	NULL	NULL	all- trans-retinoic acid receptor	GP		forms heterodimer with					9-cis-retinoic acid receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_15_13271_s_159	12540843	A model proposed for the interaction of SRC-1 with a heterodimer of the receptors for all- trans-retinoic acid and 9- cis-retinoic acid suggests that binding of tandem NR boxes occurs in a cooperative manner ( 26).	bind
42543	2	11028	6	10	NULL	NULL	NULL	SRC-1	GP		interacts with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_15_13271_s_159	12540843	A model proposed for the interaction of SRC-1 with a heterodimer of the receptors for all- trans-retinoic acid and 9- cis-retinoic acid suggests that binding of tandem NR boxes occurs in a cooperative manner ( 26).	bind
49095	1	11028	7	10	NULL	NULL	NULL	all- trans-retinoic acid receptor	GP		forms heterodimer with					9-cis-retinoic acid receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_15_13271_s_159	12540843	A model proposed for the interaction of SRC-1 with a heterodimer of the receptors for all- trans-retinoic acid and 9- cis-retinoic acid suggests that binding of tandem NR boxes occurs in a cooperative manner ( 26).	bind
49096	2	11028	7	10	NULL	NULL	NULL	SRC-1	GP		interacts with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_15_13271_s_159	12540843	A model proposed for the interaction of SRC-1 with a heterodimer of the receptors for all- trans-retinoic acid and 9- cis-retinoic acid suggests that binding of tandem NR boxes occurs in a cooperative manner ( 26).	bind
42349	1	11029	6	10	NULL	NULL	NULL	gelsolin	GP	activation of	leads to					actin cytoskeleton	CellComponent	changes in			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_103_3_347_s_257	9927495	A model showing how gelsolin activation leading to dynamic changes in the actin cytoskeleton may modify tissue injury in cerebral ischemia.	bind
42350	2	11029	6	10	NULL	NULL	NULL	statement 1	Process		modify		may			tissue injury	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_103_3_347_s_257	9927495	A model showing how gelsolin activation leading to dynamic changes in the actin cytoskeleton may modify tissue injury in cerebral ischemia.	bind
42351	3	11029	6	10	NULL	NULL	NULL	statement 2	Process		occurs during					cerebral ischemia	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_103_3_347_s_257	9927495	A model showing how gelsolin activation leading to dynamic changes in the actin cytoskeleton may modify tissue injury in cerebral ischemia.	bind
49102	1	11029	7	10	NULL	NULL	NULL	gelsolin	GP	activation of	leads to					actin cytoskeleton	CellComponent	dynamic changes in			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_103_3_347_s_257	9927495	A model showing how gelsolin activation leading to dynamic changes in the actin cytoskeleton may modify tissue injury in cerebral ischemia.	bind
49103	2	11029	7	10	NULL	NULL	NULL	statement 1	Process		modify		may			tissue injury	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_103_3_347_s_257	9927495	A model showing how gelsolin activation leading to dynamic changes in the actin cytoskeleton may modify tissue injury in cerebral ischemia.	bind
57753	3	11029	7	10	NULL	NULL	NULL	statement 2	Process		occurs during					cerebral ischemia	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_103_3_347_s_257	9927495	A model showing how gelsolin activation leading to dynamic changes in the actin cytoskeleton may modify tissue injury in cerebral ischemia.	bind
42353	1	11030	6	10	NULL	NULL	NULL	calmodulin	GP		bind					L-selectin	GP		cytoplasmic tail		NULL	resting cell 	NULL	NULL	NULL	NULL	gw60_cell_92_6_809_s_206	9529256	A model that is consistent with our current data  would suggest that calmodulin is already bound to the L-selectin cytoplasmic tail  in the resting cell and that removal of calmodulin through cell activation, or  experimentally with trifluoperazine, results in L-selectin shedding.	bind
42361	2	11030	6	10	NULL	NULL	NULL	calmodulin	GP	removal of	results in					L-selectin	GP	shedding of 			NULL		NULL	NULL	NULL	NULL	gw60_cell_92_6_809_s_206	9529256	A model that is consistent with our current data  would suggest that calmodulin is already bound to the L-selectin cytoplasmic tail  in the resting cell and that removal of calmodulin through cell activation, or  experimentally with trifluoperazine, results in L-selectin shedding.	bind
49104	1	11030	7	10	NULL	NULL	NULL	calmodulin	GP		bind					L-selectin	GP		cytoplasmic tail		NULL	resting cell	NULL	NULL	NULL	NULL	gw60_cell_92_6_809_s_206	9529256	A model that is consistent with our current data  would suggest that calmodulin is already bound to the L-selectin cytoplasmic tail  in the resting cell and that removal of calmodulin through cell activation, or  experimentally with trifluoperazine, results in L-selectin shedding.	bind
49105	2	11030	7	10	NULL	NULL	NULL	calmodulin	GP	removal of	result in					L-selectin	GP	shedding of			NULL		NULL	NULL	NULL	NULL	gw60_cell_92_6_809_s_206	9529256	A model that is consistent with our current data  would suggest that calmodulin is already bound to the L-selectin cytoplasmic tail  in the resting cell and that removal of calmodulin through cell activation, or  experimentally with trifluoperazine, results in L-selectin shedding.	bind
42364	1	11031	6	10	NULL	NULL	NULL	Shh	GP		bind					Ptc	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_12_4505_s_141	16537363	A model to explain our findings would be that binding of Shh to Ptc increases surface localization of Smo for activation of PI3-kinase and Akt.	bind
42365	2	11031	6	10	NULL	NULL	NULL	statement 1	Process		increases					Smo	GP	surface localization of 			NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_12_4505_s_141	16537363	A model to explain our findings would be that binding of Shh to Ptc increases surface localization of Smo for activation of PI3-kinase and Akt.	bind
42366	3	11031	6	10	NULL	NULL	NULL	statement 2	Process		is needed for					PI3-kinase	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_12_4505_s_141	16537363	A model to explain our findings would be that binding of Shh to Ptc increases surface localization of Smo for activation of PI3-kinase and Akt.	bind
42367	4	11031	6	10	NULL	NULL	NULL	statement 2	Process		is needed for					Akt	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_12_4505_s_141	16537363	A model to explain our findings would be that binding of Shh to Ptc increases surface localization of Smo for activation of PI3-kinase and Akt.	bind
49106	1	11031	7	10	NULL	NULL	NULL	Shh	GP		bind					Ptc	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_12_4505_s_141	16537363	A model to explain our findings would be that binding of Shh to Ptc increases surface localization of Smo for activation of PI3-kinase and Akt.	bind
49109	2	11031	7	10	NULL	NULL	NULL	statement 1	Process		increase					Smo	GP	surface localization of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_12_4505_s_141	16537363	A model to explain our findings would be that binding of Shh to Ptc increases surface localization of Smo for activation of PI3-kinase and Akt.	bind
50270	3	11031	7	10	NULL	NULL	NULL	statement 2	Process		is needed for					PI3-kinase	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_12_4505_s_141	16537363	A model to explain our findings would be that binding of Shh to Ptc increases surface localization of Smo for activation of PI3-kinase and Akt.	bind
50271	4	11031	7	10	NULL	NULL	NULL	statement 2	Process		is needed for					Akt	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_12_4505_s_141	16537363	A model to explain our findings would be that binding of Shh to Ptc increases surface localization of Smo for activation of PI3-kinase and Akt.	bind
42368	1	11032	6	10	NULL	NULL	NULL	Ndd1p	GP		activates					CLB cluster genes	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_14_1789_s_293	12865300	A model to explain the mechanism for how CLB cluster genes are activated by  Ndd1p during G2 - M, based on the finding described in this report.	bind
42369	2	11032	6	10	NULL	NULL	NULL	statement 1	Process		occurs during					G2-M	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_14_1789_s_293	12865300	A model to explain the mechanism for how CLB cluster genes are activated by  Ndd1p during G2 - M, based on the finding described in this report.	bind
49111	1	11032	7	10	NULL	NULL	NULL	Ndd1p	GP		activates					CLB cluster genes	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_14_1789_s_293	12865300	A model to explain the mechanism for how CLB cluster genes are activated by  Ndd1p during G2 - M, based on the finding described in this report.	bind
49112	2	11032	7	10	NULL	NULL	NULL	statement 1	Process		occur during					G2-M phase	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_17_14_1789_s_293	12865300	A model to explain the mechanism for how CLB cluster genes are activated by  Ndd1p during G2 - M, based on the finding described in this report.	bind
42370	1	11033	6	10	NULL	NULL	NULL	PS	GP		bind					NCT	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_39_37213_s_247	12857757	A model was proposed by Takasugi  et al. ( ), suggesting that PS binds to NCT and Aph-1, forms a stable high molecular weight complex, and then subsequently binds Pen-2, allowing for PS endoproteolysis and the final glycosylation of NCT.	bind
42371	2	11033	6	10	NULL	NULL	NULL	PS	GP		bind					Aph-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_39_37213_s_247	12857757	A model was proposed by Takasugi  et al. ( ), suggesting that PS binds to NCT and Aph-1, forms a stable high molecular weight complex, and then subsequently binds Pen-2, allowing for PS endoproteolysis and the final glycosylation of NCT.	bind
42544	3	11033	6	10	NULL	NULL	NULL	statement 1	Process		bind					Pen-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_39_37213_s_247	12857757	A model was proposed by Takasugi  et al. ( ), suggesting that PS binds to NCT and Aph-1, forms a stable high molecular weight complex, and then subsequently binds Pen-2, allowing for PS endoproteolysis and the final glycosylation of NCT.	bind
42545	4	11033	6	10	NULL	NULL	NULL	statement 2	Process		bind					Pen-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_39_37213_s_247	12857757	A model was proposed by Takasugi  et al. ( ), suggesting that PS binds to NCT and Aph-1, forms a stable high molecular weight complex, and then subsequently binds Pen-2, allowing for PS endoproteolysis and the final glycosylation of NCT.	bind
42546	5	11033	6	10	NULL	NULL	NULL	statement 3	Process		allows for					PS	GP	endoproteolysis of 			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_39_37213_s_247	12857757	A model was proposed by Takasugi  et al. ( ), suggesting that PS binds to NCT and Aph-1, forms a stable high molecular weight complex, and then subsequently binds Pen-2, allowing for PS endoproteolysis and the final glycosylation of NCT.	bind
42547	6	11033	6	10	NULL	NULL	NULL	statement 4	Process		allows for					PS	GP	endoproteolysis of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_39_37213_s_247	12857757	A model was proposed by Takasugi  et al. ( ), suggesting that PS binds to NCT and Aph-1, forms a stable high molecular weight complex, and then subsequently binds Pen-2, allowing for PS endoproteolysis and the final glycosylation of NCT.	bind
42548	7	11033	6	10	NULL	NULL	NULL	statement 3	Process		allows for					NCT	GP	glycosylation of 			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_39_37213_s_247	12857757	A model was proposed by Takasugi  et al. ( ), suggesting that PS binds to NCT and Aph-1, forms a stable high molecular weight complex, and then subsequently binds Pen-2, allowing for PS endoproteolysis and the final glycosylation of NCT.	bind
42549	8	11033	6	10	NULL	NULL	NULL	statement 4	Process		allows for					NCT	GP	glycosylation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_39_37213_s_247	12857757	A model was proposed by Takasugi  et al. ( ), suggesting that PS binds to NCT and Aph-1, forms a stable high molecular weight complex, and then subsequently binds Pen-2, allowing for PS endoproteolysis and the final glycosylation of NCT.	bind
49113	1	11033	7	10	NULL	NULL	NULL	 PS	GP		bind					NCT	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_39_37213_s_247	12857757	A model was proposed by Takasugi  et al. ( ), suggesting that PS binds to NCT and Aph-1, forms a stable high molecular weight complex, and then subsequently binds Pen-2, allowing for PS endoproteolysis and the final glycosylation of NCT.	bind
49114	2	11033	7	10	NULL	NULL	NULL	PS	GP		bind					Aph-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_39_37213_s_247	12857757	A model was proposed by Takasugi  et al. ( ), suggesting that PS binds to NCT and Aph-1, forms a stable high molecular weight complex, and then subsequently binds Pen-2, allowing for PS endoproteolysis and the final glycosylation of NCT.	bind
49115	3	11033	7	10	NULL	NULL	NULL	statement 1	Process		forms					high molecular weight complex		stable			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_39_37213_s_247	12857757	A model was proposed by Takasugi  et al. ( ), suggesting that PS binds to NCT and Aph-1, forms a stable high molecular weight complex, and then subsequently binds Pen-2, allowing for PS endoproteolysis and the final glycosylation of NCT.	bind
49116	4	11033	7	10	NULL	NULL	NULL	statement 2	Process		forms					high molecular weight complex		stable			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_39_37213_s_247	12857757	A model was proposed by Takasugi  et al. ( ), suggesting that PS binds to NCT and Aph-1, forms a stable high molecular weight complex, and then subsequently binds Pen-2, allowing for PS endoproteolysis and the final glycosylation of NCT.	bind
49117	5	11033	7	10	NULL	NULL	NULL	statement 3	Process		bind					Pen-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_39_37213_s_247	12857757	A model was proposed by Takasugi  et al. ( ), suggesting that PS binds to NCT and Aph-1, forms a stable high molecular weight complex, and then subsequently binds Pen-2, allowing for PS endoproteolysis and the final glycosylation of NCT.	bind
49118	6	11033	7	10	NULL	NULL	NULL	statement 4	Process		bind					Pen-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_39_37213_s_247	12857757	A model was proposed by Takasugi  et al. ( ), suggesting that PS binds to NCT and Aph-1, forms a stable high molecular weight complex, and then subsequently binds Pen-2, allowing for PS endoproteolysis and the final glycosylation of NCT.	bind
49119	7	11033	7	10	NULL	NULL	NULL	statement 5	Process		allows					PS	GP	endoproteolysis of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_39_37213_s_247	12857757	A model was proposed by Takasugi  et al. ( ), suggesting that PS binds to NCT and Aph-1, forms a stable high molecular weight complex, and then subsequently binds Pen-2, allowing for PS endoproteolysis and the final glycosylation of NCT.	bind
49120	8	11033	7	10	NULL	NULL	NULL	statement 6	Process		allows					PS	GP	endoproteolysis of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_39_37213_s_247	12857757	A model was proposed by Takasugi  et al. ( ), suggesting that PS binds to NCT and Aph-1, forms a stable high molecular weight complex, and then subsequently binds Pen-2, allowing for PS endoproteolysis and the final glycosylation of NCT.	bind
49121	9	11033	7	10	NULL	NULL	NULL	statement 5	Process		glycosylates					NCT	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_39_37213_s_247	12857757	A model was proposed by Takasugi  et al. ( ), suggesting that PS binds to NCT and Aph-1, forms a stable high molecular weight complex, and then subsequently binds Pen-2, allowing for PS endoproteolysis and the final glycosylation of NCT.	bind
49122	10	11033	7	10	NULL	NULL	NULL	statement 6	Process		glycosylates					NCT	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_39_37213_s_247	12857757	A model was proposed by Takasugi  et al. ( ), suggesting that PS binds to NCT and Aph-1, forms a stable high molecular weight complex, and then subsequently binds Pen-2, allowing for PS endoproteolysis and the final glycosylation of NCT.	bind
42393	1	11034	6	10	NULL	NULL	NULL	Toc 159	GP		bind					precursor protein	GP				NULL	cytosol	NULL	NULL	NULL	NULL	gw70_embo_23_3_520_s_43	14765117	A model was proposed in which Toc 159 binds to precursor proteins in the  cytosol and targets them to the membrane.	bind
42394	2	11034	6	10	NULL	NULL	NULL	precursor proteins	GP		are targeted to					membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_520_s_43	14765117	A model was proposed in which Toc 159 binds to precursor proteins in the  cytosol and targets them to the membrane.	bind
42395	3	11034	6	10	NULL	NULL	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_520_s_43	14765117	A model was proposed in which Toc 159 binds to precursor proteins in the  cytosol and targets them to the membrane.	bind
49123	1	11034	7	10	NULL	NULL	NULL	 Toc 159 	GP		bind					precursor proteins	GP				NULL	cytosol	NULL	NULL	NULL	NULL	gw70_embo_23_3_520_s_43	14765117	A model was proposed in which Toc 159 binds to precursor proteins in the  cytosol and targets them to the membrane.	bind
49124	2	11034	7	10	NULL	NULL	NULL	precursor proteins	GP		targeted to					membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_520_s_43	14765117	A model was proposed in which Toc 159 binds to precursor proteins in the  cytosol and targets them to the membrane.	bind
49125	3	11034	7	10	NULL	NULL	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_3_520_s_43	14765117	A model was proposed in which Toc 159 binds to precursor proteins in the  cytosol and targets them to the membrane.	bind
42396	1	11035	6	10	NULL	NULL	NULL	TRCF	GP		bind					RNA pol	GP	stalled			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_9_4882_s_21	7876261	A model was proposed whereby  the TRCF bound to a stalled RNA Pol, dissociated the stalled RNA  polymerase and the truncated transcript, and delivered the  A B   complex to the damage site.	bind
42397	2	11035	6	10	NULL	NULL	NULL	statement 1	Process		dissociates					RNA polymerase	GP	stalled			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_9_4882_s_21	7876261	A model was proposed whereby  the TRCF bound to a stalled RNA Pol, dissociated the stalled RNA  polymerase and the truncated transcript, and delivered the  A B   complex to the damage site.	bind
42404	3	11035	6	10	NULL	NULL	NULL	statement 1	Process		dissociates					transcript	NucleicAcid	truncated			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_9_4882_s_21	7876261	A model was proposed whereby  the TRCF bound to a stalled RNA Pol, dissociated the stalled RNA  polymerase and the truncated transcript, and delivered the  A B   complex to the damage site.	bind
42405	4	11035	6	10	NULL	NULL	NULL	A B complex	GP		is delivered to					damage site	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_9_4882_s_21	7876261	A model was proposed whereby  the TRCF bound to a stalled RNA Pol, dissociated the stalled RNA  polymerase and the truncated transcript, and delivered the  A B   complex to the damage site.	bind
42406	5	11035	6	10	NULL	NULL	NULL	statement 2	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_9_4882_s_21	7876261	A model was proposed whereby  the TRCF bound to a stalled RNA Pol, dissociated the stalled RNA  polymerase and the truncated transcript, and delivered the  A B   complex to the damage site.	bind
57754	6	11035	6	10	NULL	NULL	NULL	statement 3	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_9_4882_s_21	7876261	A model was proposed whereby  the TRCF bound to a stalled RNA Pol, dissociated the stalled RNA  polymerase and the truncated transcript, and delivered the  A B   complex to the damage site.	bind
49126	1	11035	7	10	NULL	NULL	NULL	 TRCF	GP		bind					RNA Pol	GP	stalled			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_9_4882_s_21	7876261	A model was proposed whereby  the TRCF bound to a stalled RNA Pol, dissociated the stalled RNA  polymerase and the truncated transcript, and delivered the  A B   complex to the damage site.	bind
49127	2	11035	7	10	NULL	NULL	NULL	statement 1	Process		dissociate					RNA polymerase	GP	stalled			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_9_4882_s_21	7876261	A model was proposed whereby  the TRCF bound to a stalled RNA Pol, dissociated the stalled RNA  polymerase and the truncated transcript, and delivered the  A B   complex to the damage site.	bind
49128	3	11035	7	10	NULL	NULL	NULL	statement 1	Process		dissociate					transcript	NucleicAcid	truncated			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_9_4882_s_21	7876261	A model was proposed whereby  the TRCF bound to a stalled RNA Pol, dissociated the stalled RNA  polymerase and the truncated transcript, and delivered the  A B   complex to the damage site.	bind
49129	4	11035	7	10	NULL	NULL	NULL	A B complex	GP		delivered to					damage site	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_9_4882_s_21	7876261	A model was proposed whereby  the TRCF bound to a stalled RNA Pol, dissociated the stalled RNA  polymerase and the truncated transcript, and delivered the  A B   complex to the damage site.	bind
49130	5	11035	7	10	NULL	NULL	NULL	statement 2	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_9_4882_s_21	7876261	A model was proposed whereby  the TRCF bound to a stalled RNA Pol, dissociated the stalled RNA  polymerase and the truncated transcript, and delivered the  A B   complex to the damage site.	bind
49131	6	11035	7	10	NULL	NULL	NULL	statement 3	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_9_4882_s_21	7876261	A model was proposed whereby  the TRCF bound to a stalled RNA Pol, dissociated the stalled RNA  polymerase and the truncated transcript, and delivered the  A B   complex to the damage site.	bind
42409	1	11036	6	10	NULL	NULL	NULL	RyR	GP		bind			C terminus		FKBP	GP		catalytic site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_7_5475_s_292	15591045	A model where the RyR C terminus binds the FKBP catalytic site while the N-terminal and/or central domain bind to disparate FKBP surface residues, is compatible with the three-dimensional image reconstruction of the RyR1-FKBP12 complex, which indicates that the FKBP12-binding site lies at the periphery of the cytoplasmic portion about 11 nm away from the putative channel pore ( ).	bind
42410	2	11036	6	10	NULL	NULL	NULL	RyR	GP		bind			N-terminus		FKBP surface residues	AminoAcid	disparate			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_7_5475_s_292	15591045	A model where the RyR C terminus binds the FKBP catalytic site while the N-terminal and/or central domain bind to disparate FKBP surface residues, is compatible with the three-dimensional image reconstruction of the RyR1-FKBP12 complex, which indicates that the FKBP12-binding site lies at the periphery of the cytoplasmic portion about 11 nm away from the putative channel pore ( ).	bind
42434	3	11036	6	10	NULL	NULL	NULL	RyR	GP		bind			central domain		FKBP surface residues	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_7_5475_s_292	15591045	A model where the RyR C terminus binds the FKBP catalytic site while the N-terminal and/or central domain bind to disparate FKBP surface residues, is compatible with the three-dimensional image reconstruction of the RyR1-FKBP12 complex, which indicates that the FKBP12-binding site lies at the periphery of the cytoplasmic portion about 11 nm away from the putative channel pore ( ).	bind
42435	4	11036	6	10	NULL	NULL	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_7_5475_s_292	15591045	A model where the RyR C terminus binds the FKBP catalytic site while the N-terminal and/or central domain bind to disparate FKBP surface residues, is compatible with the three-dimensional image reconstruction of the RyR1-FKBP12 complex, which indicates that the FKBP12-binding site lies at the periphery of the cytoplasmic portion about 11 nm away from the putative channel pore ( ).	bind
49132	1	11036	7	10	NULL	NULL	NULL	RyR	GP		bind			C terminus		FKBP	GP		catalytic site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_7_5475_s_292	15591045	A model where the RyR C terminus binds the FKBP catalytic site while the N-terminal and/or central domain bind to disparate FKBP surface residues, is compatible with the three-dimensional image reconstruction of the RyR1-FKBP12 complex, which indicates that the FKBP12-binding site lies at the periphery of the cytoplasmic portion about 11 nm away from the putative channel pore ( ).	bind
49133	2	11036	7	10	NULL	NULL	NULL	RyR	GP		bind			N-terminal domain		FKBP surface residues	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_7_5475_s_292	15591045	A model where the RyR C terminus binds the FKBP catalytic site while the N-terminal and/or central domain bind to disparate FKBP surface residues, is compatible with the three-dimensional image reconstruction of the RyR1-FKBP12 complex, which indicates that the FKBP12-binding site lies at the periphery of the cytoplasmic portion about 11 nm away from the putative channel pore ( ).	bind
49134	3	11036	7	10	NULL	NULL	NULL	RyR	GP		bind			central domain		FKBP surface residues	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_7_5475_s_292	15591045	A model where the RyR C terminus binds the FKBP catalytic site while the N-terminal and/or central domain bind to disparate FKBP surface residues, is compatible with the three-dimensional image reconstruction of the RyR1-FKBP12 complex, which indicates that the FKBP12-binding site lies at the periphery of the cytoplasmic portion about 11 nm away from the putative channel pore ( ).	bind
49135	4	11036	7	10	NULL	NULL	NULL	RyR1	GP		forms complex with					FKBP12	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_7_5475_s_292	15591045	A model where the RyR C terminus binds the FKBP catalytic site while the N-terminal and/or central domain bind to disparate FKBP surface residues, is compatible with the three-dimensional image reconstruction of the RyR1-FKBP12 complex, which indicates that the FKBP12-binding site lies at the periphery of the cytoplasmic portion about 11 nm away from the putative channel pore ( ).	bind
49136	5	11036	7	NULL	NULL	0	NULL		NULL		lies at	NULL		FKBP12-binding site			NULL	periphery of	cytoplasmic portion		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_7_5475_s_292	15591045	A model where the RyR C terminus binds the FKBP catalytic site while the N-terminal and/or central domain bind to disparate FKBP surface residues, is compatible with the three-dimensional image reconstruction of the RyR1-FKBP12 complex, which indicates that the FKBP12-binding site lies at the periphery of the cytoplasmic portion about 11 nm away from the putative channel pore ( ).	bind
42437	1	11037	6	10	NULL	NULL	NULL	LTA4	GP		bind					humLTA4H	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_39_33477_s_96	16024909	A modeled binding conformation of LTA4 to  humLTA4H is shown in  green.	bind
49137	1	11037	7	10	NULL	NULL	NULL	LTA4	GP		bind					humLTA4H	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_39_33477_s_96	16024909	A modeled binding conformation of LTA4 to  humLTA4H is shown in  green.	bind
42438	1	11038	6	10	NULL	NULL	NULL	p85-p110 dimer	GP		bind					IRS protein	GP	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_1_419_s_192	11752399	A moderate decrease in the amount of p85 protein (either p85alpha or p85beta) may reduce these inhibitory effects and leaves the amount of p85-p110 dimer bound to tyrosine-phosphorylated IRS proteins almost unchanged.	bind
50272	2	11038	6	10	NULL	NULL	NULL	p85alpha	GP	decrease in	does not effect					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_1_419_s_192	11752399	A moderate decrease in the amount of p85 protein (either p85alpha or p85beta) may reduce these inhibitory effects and leaves the amount of p85-p110 dimer bound to tyrosine-phosphorylated IRS proteins almost unchanged.	bind
50273	3	11038	6	10	NULL	NULL	NULL	p85beta \t	GP	decrease in	does not effect					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_1_419_s_192	11752399	A moderate decrease in the amount of p85 protein (either p85alpha or p85beta) may reduce these inhibitory effects and leaves the amount of p85-p110 dimer bound to tyrosine-phosphorylated IRS proteins almost unchanged.	bind
49139	1	11038	7	10	NULL	NULL	NULL	p85-p110 dimer	GP		bind					IRS proteins	GP	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_1_419_s_192	11752399	A moderate decrease in the amount of p85 protein (either p85alpha or p85beta) may reduce these inhibitory effects and leaves the amount of p85-p110 dimer bound to tyrosine-phosphorylated IRS proteins almost unchanged.	bind
49140	2	11038	7	10	NULL	NULL	NULL	p85alpha	GP	decrease in	does not affect					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_1_419_s_192	11752399	A moderate decrease in the amount of p85 protein (either p85alpha or p85beta) may reduce these inhibitory effects and leaves the amount of p85-p110 dimer bound to tyrosine-phosphorylated IRS proteins almost unchanged.	bind
49141	3	11038	7	10	NULL	NULL	NULL	p85beta	GP	decrease in	does not affect					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_1_419_s_192	11752399	A moderate decrease in the amount of p85 protein (either p85alpha or p85beta) may reduce these inhibitory effects and leaves the amount of p85-p110 dimer bound to tyrosine-phosphorylated IRS proteins almost unchanged.	bind
42440	1	11039	6	10	NULL	NULL	NULL	E2	GP	removal of;; bovine	increases			bilipoyl domain region		PDP	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_23_14130_s_239	9603912	A modest (40%) increase in PDP activity was observed using an E1-binding preparation of bovine E2 in which the bilipoyl domain region was selectively removed by collagenase treatment ( 11).	bind
67422	1	11039	7	10	NULL	0	NULL	E2	GP	removal of;; bovine	increases			bilipoyl domain region		PDP	GP	activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_23_14130_s_239	9603912	A modest (40%) increase in PDP activity was observed using an E1-binding preparation of bovine E2 in which the bilipoyl domain region was selectively removed by collagenase treatment ( 11).	bind
42550	1	11040	6	10	NULL	NULL	NULL	C4BP	GP		bind					protein S	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_15099_s_264	11847209	A modest inhibitory effect of HPS 34 on the C4BP binding to protein S was found only when HPS 34 and protein S were preincubated using a large molar excess of the antibody, whereas no binding of HPS 34 to the C4BP-protein S complex was detected with surface plasmon resonance.	bind
42551	2	11040	6	10	NULL	NULL	NULL	HPS34	GP		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_15099_s_264	11847209	A modest inhibitory effect of HPS 34 on the C4BP binding to protein S was found only when HPS 34 and protein S were preincubated using a large molar excess of the antibody, whereas no binding of HPS 34 to the C4BP-protein S complex was detected with surface plasmon resonance.	bind
50274	3	11040	6	10	NULL	NULL	NULL	HPS 34	GP		does not bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_15099_s_264	11847209	A modest inhibitory effect of HPS 34 on the C4BP binding to protein S was found only when HPS 34 and protein S were preincubated using a large molar excess of the antibody, whereas no binding of HPS 34 to the C4BP-protein S complex was detected with surface plasmon resonance.	bind
49142	1	11040	7	10	NULL	NULL	NULL	C4BP	GP		bind					protein S	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_15099_s_264	11847209	A modest inhibitory effect of HPS 34 on the C4BP binding to protein S was found only when HPS 34 and protein S were preincubated using a large molar excess of the antibody, whereas no binding of HPS 34 to the C4BP-protein S complex was detected with surface plasmon resonance.	bind
49143	2	11040	7	10	NULL	NULL	NULL	HPS 34	GP		inhibit		modestly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_15099_s_264	11847209	A modest inhibitory effect of HPS 34 on the C4BP binding to protein S was found only when HPS 34 and protein S were preincubated using a large molar excess of the antibody, whereas no binding of HPS 34 to the C4BP-protein S complex was detected with surface plasmon resonance.	bind
49144	3	11040	7	10	NULL	NULL	NULL	HPS 34	GP		does not bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_15099_s_264	11847209	A modest inhibitory effect of HPS 34 on the C4BP binding to protein S was found only when HPS 34 and protein S were preincubated using a large molar excess of the antibody, whereas no binding of HPS 34 to the C4BP-protein S complex was detected with surface plasmon resonance.	bind
42441	1	11041	6	10	NULL	NULL	NULL	pre-mRNA	NucleicAcid		bind					U6 snRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_11_2475_s_68	16688215	A modification at intron position +10 should therefore not interfere with pre-mRNA  binding to U6 snRNA or with spliceosome function.	bind
42442	2	11041	6	10	NULL	NULL	NULL			modification at	does not interfere				intron position +10	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_11_2475_s_68	16688215	A modification at intron position +10 should therefore not interfere with pre-mRNA  binding to U6 snRNA or with spliceosome function.	bind
42443	3	11041	6	10	NULL	NULL	NULL			modification at	does not interfere with				intron position +10	spliceosome 	NucleicAcid	function of			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_11_2475_s_68	16688215	A modification at intron position +10 should therefore not interfere with pre-mRNA  binding to U6 snRNA or with spliceosome function.	bind
49145	1	11041	7	10	NULL	NULL	NULL	pre-mRNA	NucleicAcid		bind					U6 snRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_11_2475_s_68	16688215	A modification at intron position +10 should therefore not interfere with pre-mRNA  binding to U6 snRNA or with spliceosome function.	bind
49146	2	11041	7	10	NULL	NULL	NULL			modification of	does not interfere with				intron position +10 	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_11_2475_s_68	16688215	A modification at intron position +10 should therefore not interfere with pre-mRNA  binding to U6 snRNA or with spliceosome function.	bind
49147	3	11041	7	10	NULL	NULL	NULL			modification of	does not interfere with				intron position +10 	spliceosome	Process	function of			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_11_2475_s_68	16688215	A modification at intron position +10 should therefore not interfere with pre-mRNA  binding to U6 snRNA or with spliceosome function.	bind
42444	1	11042	6	10	NULL	NULL	NULL	U11 snRNP	GP		bind					pre-mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_13_7_851_s_296	10197985	A modification of the RNase H protection assays described previously (Barabino et al. 1990  ; Eperon et al. 1993  ) was used to examine the binding of U11 and U12 snRNPs to pre-mRNA.	bind
42445	2	11042	6	10	NULL	NULL	NULL	U12 snRNP	GP		bind					pre-mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_13_7_851_s_296	10197985	A modification of the RNase H protection assays described previously (Barabino et al. 1990  ; Eperon et al. 1993  ) was used to examine the binding of U11 and U12 snRNPs to pre-mRNA.	bind
49195	1	11042	7	10	NULL	NULL	NULL	U11 snRNP	GP		bind					pre-mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_13_7_851_s_296	10197985	A modification of the RNase H protection assays described previously (Barabino et al. 1990  ; Eperon et al. 1993  ) was used to examine the binding of U11 and U12 snRNPs to pre-mRNA.	bind
49196	2	11042	7	10	NULL	NULL	NULL	U12 snRNP	GP		bind					pre-mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_13_7_851_s_296	10197985	A modification of the RNase H protection assays described previously (Barabino et al. 1990  ; Eperon et al. 1993  ) was used to examine the binding of U11 and U12 snRNPs to pre-mRNA.	bind
42446	1	11043	6	10	NULL	NULL	NULL	Cla4p	GP	GST-tagged	does not bind		specifically	CRIB domain		Cdc42p	GP	myc-tagged			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1239_s_106	11359919	A modification of this strategy was used for Cla4p because the GST-tagged Cla4p CRIB domain did not display specific binding to myc-tagged Cdc42p.	bind
49197	1	11043	7	10	NULL	NULL	NULL	 Cla4p	GP	 GST-tagged	does not bind		specifically	CRIB domain		Cdc42p	GP	myc-tagged			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_5_1239_s_106	11359919	A modification of this strategy was used for Cla4p because the GST-tagged Cla4p CRIB domain did not display specific binding to myc-tagged Cdc42p.	bind
42447	1	11044	6	10	NULL	NULL	NULL	afadin	GP		bind					p120ctn	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_24095_s_211	15857834	A modification or another protein(s) may be required for the efficient binding between afadin and p120ctn.	bind
49198	1	11044	7	10	NULL	NULL	NULL	afadin	GP		bind					p120ctn	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_24095_s_211	15857834	A modification or another protein(s) may be required for the efficient binding between afadin and p120ctn.	bind
42448	1	11045	6	10	NULL	NULL	NULL	CREB	GP		bind					mtDNA	NucleicAcid				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_pnas_102_39_13915_s_192	16169904	A modified  ChIP method was used for detection of  in vivo binding of CREB to mtDNA as described in  Materials and Methods.	bind
49199	1	11045	7	10	NULL	NULL	NULL	CREB 	GP		bind					mtDNA	NucleicAcid				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_pnas_102_39_13915_s_192	16169904	A modified  ChIP method was used for detection of  in vivo binding of CREB to mtDNA as described in  Materials and Methods.	bind
42449	1	11046	6	10	NULL	NULL	NULL	NP220	GP		bind		preferentially			dsDNA	NucleicAcid			cytidine cluster	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_21_12525_s_123	8647861	A modified  SAAB method employing the pK1 product showed that NP220 preferentially  binds to cytidine clusters in either strand of dsDNA.	bind
49200	1	11046	7	10	NULL	NULL	NULL	NP220	GP		bind		preferentially			dsDNA	NucleicAcid			cytidine clusters 	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_21_12525_s_123	8647861	A modified  SAAB method employing the pK1 product showed that NP220 preferentially  binds to cytidine clusters in either strand of dsDNA.	bind
42450	1	11047	6	10	NULL	NULL	NULL	ATP	Chemical		bind		tightly			CF(0)F(1)	GP	chloroplast	noncatalytic site		NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_photosynth-res_88_1_16440137_s_2	16440137	A modified 'cold chase'' technique was used to study tight [(14)C]ADP and  [(14)C]ATP binding to noncatalytic sites of chloroplast ATP synthase (CF(0)F(1)).	bind
42451	2	11047	6	10	NULL	NULL	NULL	ADP	Chemical		bind		tightly			CF(0)F(1)	GP	chloroplast	noncatalytic site		NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_photosynth-res_88_1_16440137_s_2	16440137	A modified 'cold chase'' technique was used to study tight [(14)C]ADP and  [(14)C]ATP binding to noncatalytic sites of chloroplast ATP synthase (CF(0)F(1)).	bind
50275	3	11047	6	10	NULL	NULL	NULL	CF(0)F(1)	GP		is a type of					ATP synthase	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_photosynth-res_88_1_16440137_s_2	16440137	A modified 'cold chase'' technique was used to study tight [(14)C]ADP and  [(14)C]ATP binding to noncatalytic sites of chloroplast ATP synthase (CF(0)F(1)).	bind
49201	1	11047	7	10	NULL	NULL	NULL	ADP	Chemical		bind		tightly			CF(0)F(1)	GP	chloroplast	noncatalytic site		NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_photosynth-res_88_1_16440137_s_2	16440137	A modified 'cold chase'' technique was used to study tight [(14)C]ADP and  [(14)C]ATP binding to noncatalytic sites of chloroplast ATP synthase (CF(0)F(1)).	bind
49202	2	11047	7	10	NULL	NULL	NULL	ATP	Chemical		bind		tightly			CF(0)F(1)	GP	chloroplast	noncatalytic site		NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_photosynth-res_88_1_16440137_s_2	16440137	A modified 'cold chase'' technique was used to study tight [(14)C]ADP and  [(14)C]ATP binding to noncatalytic sites of chloroplast ATP synthase (CF(0)F(1)).	bind
50276	3	11047	7	10	NULL	NULL	NULL	CF(0)F(1)	GP		is a type of					ATP synthase	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_photosynth-res_88_1_16440137_s_2	16440137	A modified 'cold chase'' technique was used to study tight [(14)C]ADP and  [(14)C]ATP binding to noncatalytic sites of chloroplast ATP synthase (CF(0)F(1)).	bind
42452	1	11048	6	10	NULL	NULL	NULL	Sub2p	GP		bind					RNA	NucleicAcid	nascent			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_13_2620_s_5	15192704	A modified chromatin immunoprecipitation assay that includes an RNase  step indicates that Sub2p is bound to nascent RNA, Yra1p is associated with both  RNA and DNA, and Hpr1p is associated with DNA.	bind
42453	2	11048	6	10	NULL	NULL	NULL	Yra1p	GP		associates with					RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_13_2620_s_5	15192704	A modified chromatin immunoprecipitation assay that includes an RNase  step indicates that Sub2p is bound to nascent RNA, Yra1p is associated with both  RNA and DNA, and Hpr1p is associated with DNA.	bind
42454	3	11048	6	10	NULL	NULL	NULL	Yra1p	GP		associates with					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_13_2620_s_5	15192704	A modified chromatin immunoprecipitation assay that includes an RNase  step indicates that Sub2p is bound to nascent RNA, Yra1p is associated with both  RNA and DNA, and Hpr1p is associated with DNA.	bind
42455	4	11048	6	10	NULL	NULL	NULL	Hpr1p	GP		associates with					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_13_2620_s_5	15192704	A modified chromatin immunoprecipitation assay that includes an RNase  step indicates that Sub2p is bound to nascent RNA, Yra1p is associated with both  RNA and DNA, and Hpr1p is associated with DNA.	bind
49203	1	11048	7	10	NULL	NULL	NULL	 Sub2p	GP		bind					RNA	NucleicAcid	nascent			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_13_2620_s_5	15192704	A modified chromatin immunoprecipitation assay that includes an RNase  step indicates that Sub2p is bound to nascent RNA, Yra1p is associated with both  RNA and DNA, and Hpr1p is associated with DNA.	bind
49204	2	11048	7	10	NULL	NULL	NULL	Yra1p	GP		associate with					RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_13_2620_s_5	15192704	A modified chromatin immunoprecipitation assay that includes an RNase  step indicates that Sub2p is bound to nascent RNA, Yra1p is associated with both  RNA and DNA, and Hpr1p is associated with DNA.	bind
49205	3	11048	7	10	NULL	NULL	NULL	Yra1p	GP		associate with					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_13_2620_s_5	15192704	A modified chromatin immunoprecipitation assay that includes an RNase  step indicates that Sub2p is bound to nascent RNA, Yra1p is associated with both  RNA and DNA, and Hpr1p is associated with DNA.	bind
49206	4	11048	7	10	NULL	NULL	NULL	Hpr1p	GP		associate with					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_13_2620_s_5	15192704	A modified chromatin immunoprecipitation assay that includes an RNase  step indicates that Sub2p is bound to nascent RNA, Yra1p is associated with both  RNA and DNA, and Hpr1p is associated with DNA.	bind
42456	1	11049	6	10	NULL	NULL	NULL	DPPIV	GP		bind					FN	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_27_24600_s_67	12716896	A modified enzyme-linked  immunosorbent assay (ELISA) was used to measure the binding of DPPIV to FN  fusion proteins.	bind
57755	2	11049	6	10	NULL	NULL	NULL	FN	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_27_24600_s_67	12716896	A modified enzyme-linked  immunosorbent assay (ELISA) was used to measure the binding of DPPIV to FN  fusion proteins.	bind
49207	1	11049	7	10	NULL	NULL	NULL	DPPIV	GP		bind					FN	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_27_24600_s_67	12716896	A modified enzyme-linked  immunosorbent assay (ELISA) was used to measure the binding of DPPIV to FN  fusion proteins.	bind
49208	2	11049	7	10	NULL	NULL	NULL	FN	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_27_24600_s_67	12716896	A modified enzyme-linked  immunosorbent assay (ELISA) was used to measure the binding of DPPIV to FN  fusion proteins.	bind
42552	2	11050	6	10	NULL	NULL	NULL	ER HBD	GP		is					estrogen receptor hormone-binding domain	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_13280_s_27	9582373	A modified estrogen receptor hormone-binding domain (ER HBD) containing a point mutation rendering the HBD unable to bind estrogen while retaining affinity for the synthetic ligand 4-hydroxytamoxifen (4-OH-tamoxifen) has been used to conditionally regulate heterologous proteins ( 29,  30).	bind
42553	3	11050	6	10	NULL	NULL	NULL	ER	GP	point mutant	does not bind			HBD		estrogen	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_13280_s_27	9582373	A modified estrogen receptor hormone-binding domain (ER HBD) containing a point mutation rendering the HBD unable to bind estrogen while retaining affinity for the synthetic ligand 4-hydroxytamoxifen (4-OH-tamoxifen) has been used to conditionally regulate heterologous proteins ( 29,  30).	bind
42555	1	11050	6	10	NULL	NULL	NULL	4-OH-tamoxifen	Chemical		is					4-hydroxytamoxifen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_13280_s_27	9582373	A modified estrogen receptor hormone-binding domain (ER HBD) containing a point mutation rendering the HBD unable to bind estrogen while retaining affinity for the synthetic ligand 4-hydroxytamoxifen (4-OH-tamoxifen) has been used to conditionally regulate heterologous proteins ( 29,  30).	bind
42556	5	11050	6	10	NULL	NULL	NULL	4-OH-tamoxifen	Chemical		is a type of					synthetic ligand	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_13280_s_27	9582373	A modified estrogen receptor hormone-binding domain (ER HBD) containing a point mutation rendering the HBD unable to bind estrogen while retaining affinity for the synthetic ligand 4-hydroxytamoxifen (4-OH-tamoxifen) has been used to conditionally regulate heterologous proteins ( 29,  30).	bind
42557	4	11050	6	10	NULL	NULL	NULL	ER	GP	point mutant	has affinity for			HBD		4-OH-tamoxifen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_13280_s_27	9582373	A modified estrogen receptor hormone-binding domain (ER HBD) containing a point mutation rendering the HBD unable to bind estrogen while retaining affinity for the synthetic ligand 4-hydroxytamoxifen (4-OH-tamoxifen) has been used to conditionally regulate heterologous proteins ( 29,  30).	bind
49209	1	11050	7	10	NULL	NULL	NULL	ER	GP	point mutant	does not bind			HBD		estrogen	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_13280_s_27	9582373	A modified estrogen receptor hormone-binding domain (ER HBD) containing a point mutation rendering the HBD unable to bind estrogen while retaining affinity for the synthetic ligand 4-hydroxytamoxifen (4-OH-tamoxifen) has been used to conditionally regulate heterologous proteins ( 29,  30).	bind
49211	3	11050	7	10	NULL	NULL	NULL	ER HBD	GP		is 					estrogen receptor hormone-binding domain	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_13280_s_27	9582373	A modified estrogen receptor hormone-binding domain (ER HBD) containing a point mutation rendering the HBD unable to bind estrogen while retaining affinity for the synthetic ligand 4-hydroxytamoxifen (4-OH-tamoxifen) has been used to conditionally regulate heterologous proteins ( 29,  30).	bind
49212	4	11050	7	10	NULL	NULL	NULL	4-OH-tamoxifen	Chemical		is					 4-hydroxytamoxifen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_13280_s_27	9582373	A modified estrogen receptor hormone-binding domain (ER HBD) containing a point mutation rendering the HBD unable to bind estrogen while retaining affinity for the synthetic ligand 4-hydroxytamoxifen (4-OH-tamoxifen) has been used to conditionally regulate heterologous proteins ( 29,  30).	bind
49213	5	11050	7	10	NULL	NULL	NULL	4-OH-tamoxifen	Chemical		is a type of					synthetic ligand	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_21_13280_s_27	9582373	A modified estrogen receptor hormone-binding domain (ER HBD) containing a point mutation rendering the HBD unable to bind estrogen while retaining affinity for the synthetic ligand 4-hydroxytamoxifen (4-OH-tamoxifen) has been used to conditionally regulate heterologous proteins ( 29,  30).	bind
67423	2	11050	7	10	NULL	0	NULL	ER	GP	point mutant	has affinity for			HBD		4-OH-tamoxifen	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_21_13280_s_27	9582373	A modified estrogen receptor hormone-binding domain (ER HBD) containing a point mutation rendering the HBD unable to bind estrogen while retaining affinity for the synthetic ligand 4-hydroxytamoxifen (4-OH-tamoxifen) has been used to conditionally regulate heterologous proteins ( 29,  30).	bind
42458	1	11051	6	10	NULL	NULL	NULL	IgE Ab	GP		bind					Der p 2	GP	natural;; mite			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_43_26893_s_97	9341122	A modified monoclonal RAST measured IgE Ab binding to natural mite Der p 2 and rDer p 2 (D1S) (data not shown).	bind
42459	2	11051	6	10	NULL	NULL	NULL	IgE Ab	GP		bind					rDes p 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_43_26893_s_97	9341122	A modified monoclonal RAST measured IgE Ab binding to natural mite Der p 2 and rDer p 2 (D1S) (data not shown).	bind
49217	1	11051	7	10	NULL	NULL	NULL	 IgE Ab 	GP		bind					Der p 2	GP	natural;;mite			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_43_26893_s_97	9341122	A modified monoclonal RAST measured IgE Ab binding to natural mite Der p 2 and rDer p 2 (D1S) (data not shown).	bind
49218	2	11051	7	10	NULL	NULL	NULL	IgE Ab	GP		bind					rDer p 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_43_26893_s_97	9341122	A modified monoclonal RAST measured IgE Ab binding to natural mite Der p 2 and rDer p 2 (D1S) (data not shown).	bind
42460	1	11052	6	10	NULL	NULL	NULL	hPL	GP		bind					hPRLR	GP		ECD		NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-mol-biol_358_3_16546209_s_4	16546209	A modified surface plasmon resonance method was developed to measure  the kinetics for hPL and hGH binding to the hPRLR ECD, with and without  Zn2+ and showed that hPL has about a tenfold higher affinity for the hPRLR  ECD1 than hGH.	bind
42461	2	11052	6	10	NULL	NULL	NULL	hGH	GP		bind					hPRLR	GP		ECD		NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-mol-biol_358_3_16546209_s_4	16546209	A modified surface plasmon resonance method was developed to measure  the kinetics for hPL and hGH binding to the hPRLR ECD, with and without  Zn2+ and showed that hPL has about a tenfold higher affinity for the hPRLR  ECD1 than hGH.	bind
42462	3	11052	6	10	NULL	NULL	NULL	hPL	GP		has affinity for					hPRLR	GP		ECD1		NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-mol-biol_358_3_16546209_s_4	16546209	A modified surface plasmon resonance method was developed to measure  the kinetics for hPL and hGH binding to the hPRLR ECD, with and without  Zn2+ and showed that hPL has about a tenfold higher affinity for the hPRLR  ECD1 than hGH.	bind
42463	4	11052	6	10	NULL	NULL	NULL	hGH	GP		has affinity for					hPRLR	GP		ECD1		NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-mol-biol_358_3_16546209_s_4	16546209	A modified surface plasmon resonance method was developed to measure  the kinetics for hPL and hGH binding to the hPRLR ECD, with and without  Zn2+ and showed that hPL has about a tenfold higher affinity for the hPRLR  ECD1 than hGH.	bind
42464	5	11052	6	10	NULL	NULL	NULL	statement 3	Process		is higher than					statement 4	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-mol-biol_358_3_16546209_s_4	16546209	A modified surface plasmon resonance method was developed to measure  the kinetics for hPL and hGH binding to the hPRLR ECD, with and without  Zn2+ and showed that hPL has about a tenfold higher affinity for the hPRLR  ECD1 than hGH.	bind
49219	1	11052	7	10	NULL	NULL	NULL	hPL	GP		bind					 hPRLR	GP		ECD1		NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-mol-biol_358_3_16546209_s_4	16546209	A modified surface plasmon resonance method was developed to measure  the kinetics for hPL and hGH binding to the hPRLR ECD, with and without  Zn2+ and showed that hPL has about a tenfold higher affinity for the hPRLR  ECD1 than hGH.	bind
49220	2	11052	7	10	NULL	NULL	NULL	hGH	GP		bind					hPRLR	GP		ECD1		NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-mol-biol_358_3_16546209_s_4	16546209	A modified surface plasmon resonance method was developed to measure  the kinetics for hPL and hGH binding to the hPRLR ECD, with and without  Zn2+ and showed that hPL has about a tenfold higher affinity for the hPRLR  ECD1 than hGH.	bind
49221	3	11052	7	10	NULL	NULL	NULL	statement 1	Process	affinity of	is higher than					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-mol-biol_358_3_16546209_s_4	16546209	A modified surface plasmon resonance method was developed to measure  the kinetics for hPL and hGH binding to the hPRLR ECD, with and without  Zn2+ and showed that hPL has about a tenfold higher affinity for the hPRLR  ECD1 than hGH.	bind
42465	1	11053	6	10	NULL	NULL	NULL	agonist	Chemical		bind					V1 vascular vasopressin receptor	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_annurevpharmacol_41_0_175_s_970	11264455	A molecular  model of agonist and nonpeptide antagonist binding to the human V1 vascular vasopressin receptor.	bind
42495	2	11053	6	10	NULL	NULL	NULL	nonpeptide antagonist	Chemical		bind					V1 vascular vasopressin receptor	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_annurevpharmacol_41_0_175_s_970	11264455	A molecular  model of agonist and nonpeptide antagonist binding to the human V1 vascular vasopressin receptor.	bind
49222	1	11053	7	10	NULL	NULL	NULL	agonist	Chemical		bind					 V1 vascular vasopressin receptor	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_annurevpharmacol_41_0_175_s_970	11264455	A molecular  model of agonist and nonpeptide antagonist binding to the human V1 vascular vasopressin receptor.	bind
49223	2	11053	7	10	NULL	NULL	NULL	nonpeptide antagonist	Chemical		bind					V1 vascular vasopressin receptor	GP	human			NULL		NULL	NULL	NULL	NULL	gw70_annurevpharmacol_41_0_175_s_970	11264455	A molecular  model of agonist and nonpeptide antagonist binding to the human V1 vascular vasopressin receptor.	bind
42496	1	11054	6	10	NULL	NULL	NULL	Fab ligand	GP		bind					Integrin alpha IIbbeta 3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_28_16660_s_187	7542651	A Molecular Basis for Affinity Modulation of Fab Ligand Binding to Integrin alpha IIbbeta 3.	bind
49224	1	11054	7	10	NULL	NULL	NULL	Fab Ligand 	GP		bind					Integrin alpha IIbbeta 3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_28_16660_s_187	7542651	A Molecular Basis for Affinity Modulation of Fab Ligand Binding to Integrin alpha IIbbeta 3.	bind
42498	1	11055	6	10	NULL	NULL	NULL	HERG	GP	mutant	causes					long QT syndrome	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_2_146_s_201	9933245	A molecular basis for cardiac arrhythmia:  HERG mutations cause long QT syndrome.	bind
49225	1	11055	7	10	NULL	NULL	NULL	HERG 	GP	mutant	cause					long QT syndrome	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_2_146_s_201	9933245	A molecular basis for cardiac arrhythmia:  HERG mutations cause long QT syndrome.	bind
42558	1	11056	6	10	NULL	NULL	NULL	calmodulin 	GP		bind					MOR	GP		intracellular i3 loop		NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_308_2_512_s_296	14600246	A molecular basis for the lasting regulation of basal MOR activity was suggested by our observation that calmodulin binds to the intracellular i3 loop of MOR in competition with G proteins, thereby suppressing inherent basal G protein coupling by MOR in untreated tissue (Wang et al., 1999 , 2000 , 2001b ).	bind
42559	2	11056	6	10	NULL	NULL	NULL	G protein	GP	inherent basal	couple with					MOR	GP				NULL	untreated tissue	NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_308_2_512_s_296	14600246	A molecular basis for the lasting regulation of basal MOR activity was suggested by our observation that calmodulin binds to the intracellular i3 loop of MOR in competition with G proteins, thereby suppressing inherent basal G protein coupling by MOR in untreated tissue (Wang et al., 1999 , 2000 , 2001b ).	bind
42560	3	11056	6	10	NULL	NULL	NULL	statement 1	Process		competes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_308_2_512_s_296	14600246	A molecular basis for the lasting regulation of basal MOR activity was suggested by our observation that calmodulin binds to the intracellular i3 loop of MOR in competition with G proteins, thereby suppressing inherent basal G protein coupling by MOR in untreated tissue (Wang et al., 1999 , 2000 , 2001b ).	bind
50278	4	11056	6	10	NULL	NULL	NULL	statement 3	Process		supress					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_308_2_512_s_296	14600246	A molecular basis for the lasting regulation of basal MOR activity was suggested by our observation that calmodulin binds to the intracellular i3 loop of MOR in competition with G proteins, thereby suppressing inherent basal G protein coupling by MOR in untreated tissue (Wang et al., 1999 , 2000 , 2001b ).	bind
49227	1	11056	7	10	NULL	NULL	NULL	 calmodulin	GP		bind					MOR	GP		intracellular i3 loop 		NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_308_2_512_s_296	14600246	A molecular basis for the lasting regulation of basal MOR activity was suggested by our observation that calmodulin binds to the intracellular i3 loop of MOR in competition with G proteins, thereby suppressing inherent basal G protein coupling by MOR in untreated tissue (Wang et al., 1999 , 2000 , 2001b ).	bind
49228	2	11056	7	10	NULL	NULL	NULL	MOR	GP		couple with					G protein	GP	 inherent basal			NULL	untreated tissue	NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_308_2_512_s_296	14600246	A molecular basis for the lasting regulation of basal MOR activity was suggested by our observation that calmodulin binds to the intracellular i3 loop of MOR in competition with G proteins, thereby suppressing inherent basal G protein coupling by MOR in untreated tissue (Wang et al., 1999 , 2000 , 2001b ).	bind
49229	3	11056	7	10	NULL	NULL	NULL	statement 1	Process		compete with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_308_2_512_s_296	14600246	A molecular basis for the lasting regulation of basal MOR activity was suggested by our observation that calmodulin binds to the intracellular i3 loop of MOR in competition with G proteins, thereby suppressing inherent basal G protein coupling by MOR in untreated tissue (Wang et al., 1999 , 2000 , 2001b ).	bind
49230	4	11056	7	10	NULL	NULL	NULL	statement 3	Process		suppress					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_308_2_512_s_296	14600246	A molecular basis for the lasting regulation of basal MOR activity was suggested by our observation that calmodulin binds to the intracellular i3 loop of MOR in competition with G proteins, thereby suppressing inherent basal G protein coupling by MOR in untreated tissue (Wang et al., 1999 , 2000 , 2001b ).	bind
42561	1	11057	6	10	NULL	NULL	NULL	single chain antibody	GP		is specific for					gp120	GP	highly conserved	CD4 binding site		NULL		NULL	NULL	NULL	NULL	gw60_immunity_19_3_413_s_107	14499116	A molecular conjugate containing the effector domains of the  Pseudomonas exotoxin A linked to a single chain antibody with specificity for the highly conserved CD4 binding site of gp120 (3B3:N31H/Q100eY[dsFv]-PE) is able to kill cells productively infected with diverse CCR5- and CXCR4-tropic strains of HIV while sparing uninfected cells    (Bera et al., 1998  ; Goldstein et al., 2000  ; McHugh et al., 2002  ).	bind
42562	2	11057	6	10	NULL	NULL	NULL	exotoxin A	GP	pseudomonas	is linked to			effector domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_19_3_413_s_107	14499116	A molecular conjugate containing the effector domains of the  Pseudomonas exotoxin A linked to a single chain antibody with specificity for the highly conserved CD4 binding site of gp120 (3B3:N31H/Q100eY[dsFv]-PE) is able to kill cells productively infected with diverse CCR5- and CXCR4-tropic strains of HIV while sparing uninfected cells    (Bera et al., 1998  ; Goldstein et al., 2000  ; McHugh et al., 2002  ).	bind
42563	3	11057	6	10	NULL	NULL	NULL	HIV-CCR5 strain	Organism		infect					cells 	Cell				NULL		NULL	NULL	NULL	NULL	gw60_immunity_19_3_413_s_107	14499116	A molecular conjugate containing the effector domains of the  Pseudomonas exotoxin A linked to a single chain antibody with specificity for the highly conserved CD4 binding site of gp120 (3B3:N31H/Q100eY[dsFv]-PE) is able to kill cells productively infected with diverse CCR5- and CXCR4-tropic strains of HIV while sparing uninfected cells    (Bera et al., 1998  ; Goldstein et al., 2000  ; McHugh et al., 2002  ).	bind
42564	4	11057	6	10	NULL	NULL	NULL	HIV-CXCR4 strain	Organism		infect					cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_immunity_19_3_413_s_107	14499116	A molecular conjugate containing the effector domains of the  Pseudomonas exotoxin A linked to a single chain antibody with specificity for the highly conserved CD4 binding site of gp120 (3B3:N31H/Q100eY[dsFv]-PE) is able to kill cells productively infected with diverse CCR5- and CXCR4-tropic strains of HIV while sparing uninfected cells    (Bera et al., 1998  ; Goldstein et al., 2000  ; McHugh et al., 2002  ).	bind
42565	5	11057	6	10	NULL	NULL	NULL	statement 2	Process		kills					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_19_3_413_s_107	14499116	A molecular conjugate containing the effector domains of the  Pseudomonas exotoxin A linked to a single chain antibody with specificity for the highly conserved CD4 binding site of gp120 (3B3:N31H/Q100eY[dsFv]-PE) is able to kill cells productively infected with diverse CCR5- and CXCR4-tropic strains of HIV while sparing uninfected cells    (Bera et al., 1998  ; Goldstein et al., 2000  ; McHugh et al., 2002  ).	bind
42566	6	11057	6	10	NULL	NULL	NULL	statement 2	Process		kills					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_19_3_413_s_107	14499116	A molecular conjugate containing the effector domains of the  Pseudomonas exotoxin A linked to a single chain antibody with specificity for the highly conserved CD4 binding site of gp120 (3B3:N31H/Q100eY[dsFv]-PE) is able to kill cells productively infected with diverse CCR5- and CXCR4-tropic strains of HIV while sparing uninfected cells    (Bera et al., 1998  ; Goldstein et al., 2000  ; McHugh et al., 2002  ).	bind
49231	1	11057	7	10	NULL	NULL	NULL	molecular conjugate			contains					exotoxin A	GP	Pseudomonas	 effector domains		NULL		NULL	NULL	NULL	NULL	gw60_immunity_19_3_413_s_107	14499116	A molecular conjugate containing the effector domains of the  Pseudomonas exotoxin A linked to a single chain antibody with specificity for the highly conserved CD4 binding site of gp120 (3B3:N31H/Q100eY[dsFv]-PE) is able to kill cells productively infected with diverse CCR5- and CXCR4-tropic strains of HIV while sparing uninfected cells    (Bera et al., 1998  ; Goldstein et al., 2000  ; McHugh et al., 2002  ).	bind
49232	2	11057	7	10	NULL	NULL	NULL	statement 1	Process		linked to					single chain antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_19_3_413_s_107	14499116	A molecular conjugate containing the effector domains of the  Pseudomonas exotoxin A linked to a single chain antibody with specificity for the highly conserved CD4 binding site of gp120 (3B3:N31H/Q100eY[dsFv]-PE) is able to kill cells productively infected with diverse CCR5- and CXCR4-tropic strains of HIV while sparing uninfected cells    (Bera et al., 1998  ; Goldstein et al., 2000  ; McHugh et al., 2002  ).	bind
49233	3	11057	7	10	NULL	NULL	NULL	statement 2	Process		is specific for					gp120	GP		conserved CD4 binding site		NULL		NULL	NULL	NULL	NULL	gw60_immunity_19_3_413_s_107	14499116	A molecular conjugate containing the effector domains of the  Pseudomonas exotoxin A linked to a single chain antibody with specificity for the highly conserved CD4 binding site of gp120 (3B3:N31H/Q100eY[dsFv]-PE) is able to kill cells productively infected with diverse CCR5- and CXCR4-tropic strains of HIV while sparing uninfected cells    (Bera et al., 1998  ; Goldstein et al., 2000  ; McHugh et al., 2002  ).	bind
49234	4	11057	7	10	NULL	NULL	NULL	cells	Cell		infected with					HIV CCR5-tropic strains 	Organism				NULL		NULL	NULL	NULL	NULL	gw60_immunity_19_3_413_s_107	14499116	A molecular conjugate containing the effector domains of the  Pseudomonas exotoxin A linked to a single chain antibody with specificity for the highly conserved CD4 binding site of gp120 (3B3:N31H/Q100eY[dsFv]-PE) is able to kill cells productively infected with diverse CCR5- and CXCR4-tropic strains of HIV while sparing uninfected cells    (Bera et al., 1998  ; Goldstein et al., 2000  ; McHugh et al., 2002  ).	bind
49235	5	11057	7	10	NULL	NULL	NULL	cells	Cell		infected with					HIV CXCR4-tropic strains	Organism				NULL		NULL	NULL	NULL	NULL	gw60_immunity_19_3_413_s_107	14499116	A molecular conjugate containing the effector domains of the  Pseudomonas exotoxin A linked to a single chain antibody with specificity for the highly conserved CD4 binding site of gp120 (3B3:N31H/Q100eY[dsFv]-PE) is able to kill cells productively infected with diverse CCR5- and CXCR4-tropic strains of HIV while sparing uninfected cells    (Bera et al., 1998  ; Goldstein et al., 2000  ; McHugh et al., 2002  ).	bind
49236	6	11057	7	10	NULL	NULL	NULL	statement 3	Process		kills					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_19_3_413_s_107	14499116	A molecular conjugate containing the effector domains of the  Pseudomonas exotoxin A linked to a single chain antibody with specificity for the highly conserved CD4 binding site of gp120 (3B3:N31H/Q100eY[dsFv]-PE) is able to kill cells productively infected with diverse CCR5- and CXCR4-tropic strains of HIV while sparing uninfected cells    (Bera et al., 1998  ; Goldstein et al., 2000  ; McHugh et al., 2002  ).	bind
49237	7	11057	7	10	NULL	NULL	NULL	statement 3	Process		kills					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_19_3_413_s_107	14499116	A molecular conjugate containing the effector domains of the  Pseudomonas exotoxin A linked to a single chain antibody with specificity for the highly conserved CD4 binding site of gp120 (3B3:N31H/Q100eY[dsFv]-PE) is able to kill cells productively infected with diverse CCR5- and CXCR4-tropic strains of HIV while sparing uninfected cells    (Bera et al., 1998  ; Goldstein et al., 2000  ; McHugh et al., 2002  ).	bind
42499	1	11058	6	10	NULL	NULL	NULL	YidC	GP		bind		directly			SecDF protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_166_6_769_s_65	15364957	A molecular interaction with the Sec translocase has been found; this interaction is likely due to a direct binding of YidC to the accessory SecDF proteins ( ).	bind
42500	2	11058	6	10	NULL	NULL	NULL	SecDF	GP		is a type of					accessory protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_166_6_769_s_65	15364957	A molecular interaction with the Sec translocase has been found; this interaction is likely due to a direct binding of YidC to the accessory SecDF proteins ( ).	bind
49238	1	11058	7	10	NULL	NULL	NULL	YidC	GP		bind		directly			SecDF protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_166_6_769_s_65	15364957	A molecular interaction with the Sec translocase has been found; this interaction is likely due to a direct binding of YidC to the accessory SecDF proteins ( ).	bind
50279	2	11058	7	10	NULL	NULL	NULL	SecDF 	GP		is a type of					accessory protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_166_6_769_s_65	15364957	A molecular interaction with the Sec translocase has been found; this interaction is likely due to a direct binding of YidC to the accessory SecDF proteins ( ).	bind
42570	1	11059	6	10	NULL	NULL	NULL	PDZ domain-containing proteins 	GP		bind					EphB2	GP		C-termini		NULL		NULL	NULL	NULL	NULL	gw60_neuron_26_2_417_s_5	10839360	A molecular link to fluid regulation is provided by demonstrating that PDZ domain-containing proteins that bind the C termini of EphB2 and B-ephrins can also recognize the cytoplasmic tails of anion exchangers and aquaporins.	bind
42571	2	11059	6	10	NULL	NULL	NULL	PDZ domain-containing proteins	GP		bind					B-ephrin	GP		C-termini		NULL		NULL	NULL	NULL	NULL	gw60_neuron_26_2_417_s_5	10839360	A molecular link to fluid regulation is provided by demonstrating that PDZ domain-containing proteins that bind the C termini of EphB2 and B-ephrins can also recognize the cytoplasmic tails of anion exchangers and aquaporins.	bind
42572	3	11059	6	10	NULL	NULL	NULL	PDZ domain-containing proteins	GP		recognize					anion exchangers	GP		cytoplasmic tail		NULL		NULL	NULL	NULL	NULL	gw60_neuron_26_2_417_s_5	10839360	A molecular link to fluid regulation is provided by demonstrating that PDZ domain-containing proteins that bind the C termini of EphB2 and B-ephrins can also recognize the cytoplasmic tails of anion exchangers and aquaporins.	bind
42573	4	11059	6	10	NULL	NULL	NULL	PDZ domain-containing proteins	GP		recognize					aquaporins	GP		cytoplasmic tail		NULL		NULL	NULL	NULL	NULL	gw60_neuron_26_2_417_s_5	10839360	A molecular link to fluid regulation is provided by demonstrating that PDZ domain-containing proteins that bind the C termini of EphB2 and B-ephrins can also recognize the cytoplasmic tails of anion exchangers and aquaporins.	bind
49239	1	11059	7	10	NULL	NULL	NULL	PDZ domain-containing proteins	GP		bind					EphB2	GP		C termini		NULL		NULL	NULL	NULL	NULL	gw60_neuron_26_2_417_s_5	10839360	A molecular link to fluid regulation is provided by demonstrating that PDZ domain-containing proteins that bind the C termini of EphB2 and B-ephrins can also recognize the cytoplasmic tails of anion exchangers and aquaporins.	bind
49240	2	11059	7	10	NULL	NULL	NULL	PDZ domain-containing proteins	GP		bind					B-ephrins	GP		C termini		NULL		NULL	NULL	NULL	NULL	gw60_neuron_26_2_417_s_5	10839360	A molecular link to fluid regulation is provided by demonstrating that PDZ domain-containing proteins that bind the C termini of EphB2 and B-ephrins can also recognize the cytoplasmic tails of anion exchangers and aquaporins.	bind
49241	3	11059	7	10	NULL	NULL	NULL	PDZ domain-containing proteins	GP		recognize					anion exchangers	GP		cytoplasmic tails 		NULL		NULL	NULL	NULL	NULL	gw60_neuron_26_2_417_s_5	10839360	A molecular link to fluid regulation is provided by demonstrating that PDZ domain-containing proteins that bind the C termini of EphB2 and B-ephrins can also recognize the cytoplasmic tails of anion exchangers and aquaporins.	bind
49242	4	11059	7	10	NULL	NULL	NULL	PDZ domain-containing proteins	GP		recognize					aquaporins	GP		cytoplasmic tails		NULL		NULL	NULL	NULL	NULL	gw60_neuron_26_2_417_s_5	10839360	A molecular link to fluid regulation is provided by demonstrating that PDZ domain-containing proteins that bind the C termini of EphB2 and B-ephrins can also recognize the cytoplasmic tails of anion exchangers and aquaporins.	bind
57859	1	11060	6	10	NULL	NULL	NULL	thrombin Met-SC(1 325) complex \t	GP		undergoes					dimerization	Process				NULL	solution	NULL	NULL	NULL	NULL	gw70_nature_425_6957_535_s_53	14523451	A molecular mass of 155   10 kDa was determined for the thrombin Met-SC(1 325) complex by using sedimentation equilibrium, indicating that the complex  dimerizes in solution.	bind
49243	1	11060	7	10	NULL	NULL	NULL	thrombin Met-SC(1 325) complex 	GP		undergoes					dimerization	Process				NULL	solution	NULL	NULL	NULL	NULL	gw70_nature_425_6957_535_s_53	14523451	A molecular mass of 155   10 kDa was determined for the thrombin Met-SC(1 325) complex by using sedimentation equilibrium, indicating that the complex  dimerizes in solution.	bind
42574	1	11061	6	10	NULL	NULL	NULL	imidazole group	Chemical		bind					Cu(II) ion	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_5_2042_s_237	10051591	A molecular model constructed for the Cu4[PrP(58-91)] complex showed that the four-copper atom cluster could be accommodated without strain at the corners of a distorted tetrahedron, with two imidazole groups bound to each Cu(II) ion at adjacent coordination sites.	bind
49244	1	11061	7	10	NULL	NULL	NULL	imidazole groups	Chemical		bind					Cu(II) ion	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_5_2042_s_237	10051591	A molecular model constructed for the Cu4[PrP(58-91)] complex showed that the four-copper atom cluster could be accommodated without strain at the corners of a distorted tetrahedron, with two imidazole groups bound to each Cu(II) ion at adjacent coordination sites.	bind
42575	1	11062	6	10	NULL	NULL	NULL	agonist	Chemical		bind					V1 vascular vasopressin receptor	GP	human			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-pharmacol-exp-ther_294_1_10871312_s_1	10871312	A molecular model of agonist and nonpeptide antagonist binding to the human V(1) vascular vasopressin receptor..	bind
42576	2	11062	6	10	NULL	NULL	NULL	nonpeptide antagonist	Chemical		bind					V1 vascular vasopressin receptor	GP	human			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-pharmacol-exp-ther_294_1_10871312_s_1	10871312	A molecular model of agonist and nonpeptide antagonist binding to the human V(1) vascular vasopressin receptor..	bind
49246	1	11062	7	10	NULL	NULL	NULL	agonist	Chemical		bind					V(1) vascular vasopressin receptor	GP	human			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-pharmacol-exp-ther_294_1_10871312_s_1	10871312	A molecular model of agonist and nonpeptide antagonist binding to the human V(1) vascular vasopressin receptor..	bind
49247	2	11062	7	10	NULL	NULL	NULL	nonpeptide antagonist	Chemical		bind					V(1) vascular vasopressin receptor	GP	human			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-pharmacol-exp-ther_294_1_10871312_s_1	10871312	A molecular model of agonist and nonpeptide antagonist binding to the human V(1) vascular vasopressin receptor..	bind
42577	1	11067	6	10	NULL	NULL	NULL	Sic1	GP		bind			inhibitory domain		Cdk2-cyclin A complex	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_biochem-j_387_pt-3_15649124_s_6	15649124	A molecular model of the inhibitory domain of Sic1 bound to the Cdk2-cyclin  A complex suggested that the yeast inhibitor might productively interface  with the mammalian Cdk2-cyclin A complex.	bind
42578	2	11067	6	10	NULL	NULL	NULL	inhibitor	GP	yeast	interface with		might;;productively 			Cdk2-cyclin A complex	GP	mammalian			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_biochem-j_387_pt-3_15649124_s_6	15649124	A molecular model of the inhibitory domain of Sic1 bound to the Cdk2-cyclin  A complex suggested that the yeast inhibitor might productively interface  with the mammalian Cdk2-cyclin A complex.	bind
49248	1	11067	7	10	NULL	NULL	NULL	Sic1	GP		bind			inhibitory domain		Cdk2-cyclin A complex	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_biochem-j_387_pt-3_15649124_s_6	15649124	A molecular model of the inhibitory domain of Sic1 bound to the Cdk2-cyclin  A complex suggested that the yeast inhibitor might productively interface  with the mammalian Cdk2-cyclin A complex.	bind
49249	2	11067	7	10	NULL	NULL	NULL	 inhibitor	GP	yeast	interface with		may;;productively			Cdk2-cyclin A complex	GP	mammalian			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_biochem-j_387_pt-3_15649124_s_6	15649124	A molecular model of the inhibitory domain of Sic1 bound to the Cdk2-cyclin  A complex suggested that the yeast inhibitor might productively interface  with the mammalian Cdk2-cyclin A complex.	bind
49250	3	11067	7	10	NULL	NULL	NULL	statement 1	Process		suggest					statement 2	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_biochem-j_387_pt-3_15649124_s_6	15649124	A molecular model of the inhibitory domain of Sic1 bound to the Cdk2-cyclin  A complex suggested that the yeast inhibitor might productively interface  with the mammalian Cdk2-cyclin A complex.	bind
42579	1	11068	6	10	NULL	NULL	NULL	anti-Abeta IgG 	GP		bind					Abeta fibrils	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_bioorg-med-chem-lett_16_4_16290147_s_6	16290147	A molecular surface coating with 3,6-diamino acridine  was able to inhibit 76+/-10% of the binding of an anti-Abeta IgG to Abeta  fibrils.	bind
42580	2	11068	6	10	NULL	NULL	NULL	3,6-diamino acridine 	Chemical		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_bioorg-med-chem-lett_16_4_16290147_s_6	16290147	A molecular surface coating with 3,6-diamino acridine  was able to inhibit 76+/-10% of the binding of an anti-Abeta IgG to Abeta  fibrils.	bind
49251	1	11068	7	10	NULL	NULL	NULL	anti-Abeta IgG	GP		bind					Abeta fibrils	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_bioorg-med-chem-lett_16_4_16290147_s_6	16290147	A molecular surface coating with 3,6-diamino acridine  was able to inhibit 76+/-10% of the binding of an anti-Abeta IgG to Abeta  fibrils.	bind
49252	2	11068	7	10	NULL	NULL	NULL	 3,6-diamino acridine	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_bioorg-med-chem-lett_16_4_16290147_s_6	16290147	A molecular surface coating with 3,6-diamino acridine  was able to inhibit 76+/-10% of the binding of an anti-Abeta IgG to Abeta  fibrils.	bind
42581	1	11069	6	10	NULL	NULL	NULL	PPS	Chemical		is					3-(1-pyridino)-1-propanesulfonate	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_26_27511_s_151	15075327	A molecule of 3-(1-pyridino)-1-propanesulfonate (PPS) is bound to Stx2 in four of the five potential type 1 binding sites.	bind
42582	2	11069	6	10	NULL	NULL	NULL	PPS	Chemical		bind					Stx2	GP		type 1 binding site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_26_27511_s_151	15075327	A molecule of 3-(1-pyridino)-1-propanesulfonate (PPS) is bound to Stx2 in four of the five potential type 1 binding sites.	bind
49253	1	11069	7	10	NULL	NULL	NULL	PPS	Chemical		bind					Stx2	GP		type 1 binding site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_26_27511_s_151	15075327	A molecule of 3-(1-pyridino)-1-propanesulfonate (PPS) is bound to Stx2 in four of the five potential type 1 binding sites.	bind
49254	2	11069	7	10	NULL	NULL	NULL	PPS	Chemical		is					3-(1-pyridino)-1-propanesulfonate	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_26_27511_s_151	15075327	A molecule of 3-(1-pyridino)-1-propanesulfonate (PPS) is bound to Stx2 in four of the five potential type 1 binding sites.	bind
42583	1	11070	6	10	NULL	NULL	NULL	acetoacetyl-CoA	Chemical		bind					enoyl-CoA hydratase	GP				NULL		NULL	NULL	NULL	NULL	gw60_structure_6_8_957_s_107	9739087	A molecule of acetoacetyl-CoA, as it binds to enoyl-CoA hydratase  [17]  , is shown in ball-and-stick representation (green).	bind
49255	1	11070	7	10	NULL	NULL	NULL	acetoacetyl-CoA	Chemical		bind					enoyl-CoA hydratase	GP				NULL		NULL	NULL	NULL	NULL	gw60_structure_6_8_957_s_107	9739087	A molecule of acetoacetyl-CoA, as it binds to enoyl-CoA hydratase  [17]  , is shown in ball-and-stick representation (green).	bind
42845	1	11071	6	10	NULL	NULL	NULL	cAMP	Chemical		bind								B domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_42_35521_s_201	16109722	A molecule of cAMP must first bind to the B domain, allowing cAMP binding to the A domain, which then causes the conformational changes directly responsible for C subunit activation.	bind
42846	2	11071	6	10	NULL	NULL	NULL	cAMP	Chemical		bind								A domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_42_35521_s_201	16109722	A molecule of cAMP must first bind to the B domain, allowing cAMP binding to the A domain, which then causes the conformational changes directly responsible for C subunit activation.	bind
42847	3	11071	6	10	NULL	NULL	NULL	statement 1	Process		allows					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_42_35521_s_201	16109722	A molecule of cAMP must first bind to the B domain, allowing cAMP binding to the A domain, which then causes the conformational changes directly responsible for C subunit activation.	bind
42848	4	11071	6	10	NULL	NULL	NULL	statement 2	Process		leads to					conformational changes	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_42_35521_s_201	16109722	A molecule of cAMP must first bind to the B domain, allowing cAMP binding to the A domain, which then causes the conformational changes directly responsible for C subunit activation.	bind
42849	5	11071	6	10	NULL	NULL	NULL	statement 4	Process		is responsible for		directly			C subunit	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_42_35521_s_201	16109722	A molecule of cAMP must first bind to the B domain, allowing cAMP binding to the A domain, which then causes the conformational changes directly responsible for C subunit activation.	bind
49256	1	11071	7	10	NULL	NULL	NULL	cAMP	Chemical		bind								B domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_42_35521_s_201	16109722	A molecule of cAMP must first bind to the B domain, allowing cAMP binding to the A domain, which then causes the conformational changes directly responsible for C subunit activation.	bind
49257	2	11071	7	10	NULL	NULL	NULL	cAMP	Chemical		bind								A domain		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_42_35521_s_201	16109722	A molecule of cAMP must first bind to the B domain, allowing cAMP binding to the A domain, which then causes the conformational changes directly responsible for C subunit activation.	bind
49258	3	11071	7	10	NULL	NULL	NULL	statement 1	Process		allows 					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_42_35521_s_201	16109722	A molecule of cAMP must first bind to the B domain, allowing cAMP binding to the A domain, which then causes the conformational changes directly responsible for C subunit activation.	bind
49259	4	11071	7	10	NULL	NULL	NULL	statement 2	Process		cause					conformational changes	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_42_35521_s_201	16109722	A molecule of cAMP must first bind to the B domain, allowing cAMP binding to the A domain, which then causes the conformational changes directly responsible for C subunit activation.	bind
49260	5	11071	7	10	NULL	NULL	NULL	statement 4	Process		leads to		directly			C subunit	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_42_35521_s_201	16109722	A molecule of cAMP must first bind to the B domain, allowing cAMP binding to the A domain, which then causes the conformational changes directly responsible for C subunit activation.	bind
42620	1	11072	6	10	NULL	NULL	NULL	CR1	GP	mouse	bind		less efficiency	SCR		C3b	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-immunol_153_2_8021513_s_6	8021513	A molecule that contains only the  first six SCRs of mouse CR1 also binds C3b, but with less efficiency.	bind
49261	1	11072	7	10	NULL	NULL	NULL	CR1	GP	mouse	bind		less efficiency	SCRs		C3b	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-immunol_153_2_8021513_s_6	8021513	A molecule that contains only the  first six SCRs of mouse CR1 also binds C3b, but with less efficiency.	bind
42621	1	11074	6	10	NULL	NULL	NULL	mAb2G5	GP		is a type of					monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_97_6_755_s_32	10380927	A monoclonal  antibody, mAb2G5, which recognizes a region close to the ATP-binding cleft of the N-terminal  DnaK domain (Krska et al., 1993   ), coprecipitated DnaK and a wide variety  of newly synthesized polypeptides from the lysed spheroplasts (  Figure 1A, lane 3).	bind
42625	2	11074	6	10	NULL	NULL	NULL	mAb2G5	GP		recognizes								ATP-binding cleft of the N-terminal DnaK domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_97_6_755_s_32	10380927	A monoclonal  antibody, mAb2G5, which recognizes a region close to the ATP-binding cleft of the N-terminal  DnaK domain (Krska et al., 1993   ), coprecipitated DnaK and a wide variety  of newly synthesized polypeptides from the lysed spheroplasts (  Figure 1A, lane 3).	bind
42626	3	11074	6	10	NULL	NULL	NULL	mAb2G5	GP		bind					DnaK	GP				NULL	lysed spheroplasts	NULL	NULL	NULL	NULL	gw60_cell_97_6_755_s_32	10380927	A monoclonal  antibody, mAb2G5, which recognizes a region close to the ATP-binding cleft of the N-terminal  DnaK domain (Krska et al., 1993   ), coprecipitated DnaK and a wide variety  of newly synthesized polypeptides from the lysed spheroplasts (  Figure 1A, lane 3).	bind
49262	1	11074	7	10	NULL	NULL	NULL	mAb2G5	GP		recognizes							region close to	 ATP-binding cleft of the N-terminal DnaK domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_97_6_755_s_32	10380927	A monoclonal  antibody, mAb2G5, which recognizes a region close to the ATP-binding cleft of the N-terminal  DnaK domain (Krska et al., 1993   ), coprecipitated DnaK and a wide variety  of newly synthesized polypeptides from the lysed spheroplasts (  Figure 1A, lane 3).	bind
49263	2	11074	7	10	NULL	NULL	NULL	statement 1	Process		bind					DnaK	GP				NULL	lysed spheroplasts	NULL	NULL	NULL	NULL	gw60_cell_97_6_755_s_32	10380927	A monoclonal  antibody, mAb2G5, which recognizes a region close to the ATP-binding cleft of the N-terminal  DnaK domain (Krska et al., 1993   ), coprecipitated DnaK and a wide variety  of newly synthesized polypeptides from the lysed spheroplasts (  Figure 1A, lane 3).	bind
49264	3	11074	7	10	NULL	NULL	NULL	statement 1	Process		bind					polypeptides	AminoAcid	newly synthesized			NULL	lysed spheroplasts	NULL	NULL	NULL	NULL	gw60_cell_97_6_755_s_32	10380927	A monoclonal  antibody, mAb2G5, which recognizes a region close to the ATP-binding cleft of the N-terminal  DnaK domain (Krska et al., 1993   ), coprecipitated DnaK and a wide variety  of newly synthesized polypeptides from the lysed spheroplasts (  Figure 1A, lane 3).	bind
49265	4	11074	7	10	NULL	NULL	NULL	mAb2G5	GP		is a type of					monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_97_6_755_s_32	10380927	A monoclonal  antibody, mAb2G5, which recognizes a region close to the ATP-binding cleft of the N-terminal  DnaK domain (Krska et al., 1993   ), coprecipitated DnaK and a wide variety  of newly synthesized polypeptides from the lysed spheroplasts (  Figure 1A, lane 3).	bind
42850	1	11075	6	10	NULL	NULL	NULL	C-19	GP		is a type of					polyclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_5802_s_151	14597617	A monoclonal antibody (AB-1) whose epitope maps within amino acid residues 58 - 77 of human p21 near the CDK2 binding site and a polyclonal antibody (C-19) that binds to the C terminus of p21 and cannot recognize p21 bound to PCNA were used ( ).	bind
42851	2	11075	6	10	NULL	NULL	NULL	C-19	GP		bind					p21	GP		C terminus		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_5802_s_151	14597617	A monoclonal antibody (AB-1) whose epitope maps within amino acid residues 58 - 77 of human p21 near the CDK2 binding site and a polyclonal antibody (C-19) that binds to the C terminus of p21 and cannot recognize p21 bound to PCNA were used ( ).	bind
50280	3	11075	6	10	NULL	NULL	NULL	p21	GP		bind					PCNA	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_5802_s_151	14597617	A monoclonal antibody (AB-1) whose epitope maps within amino acid residues 58 - 77 of human p21 near the CDK2 binding site and a polyclonal antibody (C-19) that binds to the C terminus of p21 and cannot recognize p21 bound to PCNA were used ( ).	bind
57860	4	11075	6	10	NULL	NULL	NULL	AB-1	GP		is a type of					monoclonal antibody \t	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_5802_s_151	14597617	A monoclonal antibody (AB-1) whose epitope maps within amino acid residues 58 - 77 of human p21 near the CDK2 binding site and a polyclonal antibody (C-19) that binds to the C terminus of p21 and cannot recognize p21 bound to PCNA were used ( ).	bind
49266	1	11075	7	10	NULL	NULL	NULL	C-19	GP		bind					p21	GP		C terminus		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_5802_s_151	14597617	A monoclonal antibody (AB-1) whose epitope maps within amino acid residues 58 - 77 of human p21 near the CDK2 binding site and a polyclonal antibody (C-19) that binds to the C terminus of p21 and cannot recognize p21 bound to PCNA were used ( ).	bind
49267	2	11075	7	10	NULL	NULL	NULL	p21	GP		bind					PCNA	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_5802_s_151	14597617	A monoclonal antibody (AB-1) whose epitope maps within amino acid residues 58 - 77 of human p21 near the CDK2 binding site and a polyclonal antibody (C-19) that binds to the C terminus of p21 and cannot recognize p21 bound to PCNA were used ( ).	bind
49268	3	11075	7	10	NULL	NULL	NULL	C-19	GP		is a type of					polyclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_5802_s_151	14597617	A monoclonal antibody (AB-1) whose epitope maps within amino acid residues 58 - 77 of human p21 near the CDK2 binding site and a polyclonal antibody (C-19) that binds to the C terminus of p21 and cannot recognize p21 bound to PCNA were used ( ).	bind
49269	4	11075	7	10	NULL	NULL	NULL	AB-1	GP		is a type of					monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_5802_s_151	14597617	A monoclonal antibody (AB-1) whose epitope maps within amino acid residues 58 - 77 of human p21 near the CDK2 binding site and a polyclonal antibody (C-19) that binds to the C terminus of p21 and cannot recognize p21 bound to PCNA were used ( ).	bind
42852	1	11076	6	10	NULL	NULL	NULL	125I-Fn	GP		bind					M. tuberculosis	Organism				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_3_1287_s_5	11854212	A monoclonal antibody (MAb) specific to the heparin binding domain (HBD) of Fn decreases 125I-Fn binding to  M. tuberculosis; whereas MAbs specific to either the cell binding domain (CBD) or the gelatin binding domain (GBD) have no effect on Fn binding to  M. tuberculosis.	bind
42853	2	11076	6	10	NULL	NULL	NULL	MAb	GP		is specific for					Fn	GP		HBD		NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_3_1287_s_5	11854212	A monoclonal antibody (MAb) specific to the heparin binding domain (HBD) of Fn decreases 125I-Fn binding to  M. tuberculosis; whereas MAbs specific to either the cell binding domain (CBD) or the gelatin binding domain (GBD) have no effect on Fn binding to  M. tuberculosis.	bind
42854	3	11076	6	10	NULL	NULL	NULL	statement 2	Process		decreases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_3_1287_s_5	11854212	A monoclonal antibody (MAb) specific to the heparin binding domain (HBD) of Fn decreases 125I-Fn binding to  M. tuberculosis; whereas MAbs specific to either the cell binding domain (CBD) or the gelatin binding domain (GBD) have no effect on Fn binding to  M. tuberculosis.	bind
42855	4	11076	6	10	NULL	NULL	NULL	MAb	GP		is					monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_3_1287_s_5	11854212	A monoclonal antibody (MAb) specific to the heparin binding domain (HBD) of Fn decreases 125I-Fn binding to  M. tuberculosis; whereas MAbs specific to either the cell binding domain (CBD) or the gelatin binding domain (GBD) have no effect on Fn binding to  M. tuberculosis.	bind
42856	5	11076	6	10	NULL	NULL	NULL	HBD	AminoAcid		is					heparin binding domain	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_3_1287_s_5	11854212	A monoclonal antibody (MAb) specific to the heparin binding domain (HBD) of Fn decreases 125I-Fn binding to  M. tuberculosis; whereas MAbs specific to either the cell binding domain (CBD) or the gelatin binding domain (GBD) have no effect on Fn binding to  M. tuberculosis.	bind
42857	6	11076	6	10	NULL	NULL	NULL	MAb	GP		is specific for					Fn	GP		CBD		NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_3_1287_s_5	11854212	A monoclonal antibody (MAb) specific to the heparin binding domain (HBD) of Fn decreases 125I-Fn binding to  M. tuberculosis; whereas MAbs specific to either the cell binding domain (CBD) or the gelatin binding domain (GBD) have no effect on Fn binding to  M. tuberculosis.	bind
42858	7	11076	6	10	NULL	NULL	NULL	MAb	GP		is specific for					Fn	GP		GBD		NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_3_1287_s_5	11854212	A monoclonal antibody (MAb) specific to the heparin binding domain (HBD) of Fn decreases 125I-Fn binding to  M. tuberculosis; whereas MAbs specific to either the cell binding domain (CBD) or the gelatin binding domain (GBD) have no effect on Fn binding to  M. tuberculosis.	bind
42859	8	11076	6	10	NULL	NULL	NULL	statement 6	Process		has no effect on					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_3_1287_s_5	11854212	A monoclonal antibody (MAb) specific to the heparin binding domain (HBD) of Fn decreases 125I-Fn binding to  M. tuberculosis; whereas MAbs specific to either the cell binding domain (CBD) or the gelatin binding domain (GBD) have no effect on Fn binding to  M. tuberculosis.	bind
42860	9	11076	6	10	NULL	NULL	NULL	statement 7	Process		has no effect on					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_3_1287_s_5	11854212	A monoclonal antibody (MAb) specific to the heparin binding domain (HBD) of Fn decreases 125I-Fn binding to  M. tuberculosis; whereas MAbs specific to either the cell binding domain (CBD) or the gelatin binding domain (GBD) have no effect on Fn binding to  M. tuberculosis.	bind
49270	1	11076	7	10	NULL	NULL	NULL	125I-Fn	GP		bind					M. tuberculosis	Organism				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_3_1287_s_5	11854212	A monoclonal antibody (MAb) specific to the heparin binding domain (HBD) of Fn decreases 125I-Fn binding to  M. tuberculosis; whereas MAbs specific to either the cell binding domain (CBD) or the gelatin binding domain (GBD) have no effect on Fn binding to  M. tuberculosis.	bind
49271	2	11076	7	10	NULL	NULL	NULL	FnMAb	GP		decrease			HBD		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_3_1287_s_5	11854212	A monoclonal antibody (MAb) specific to the heparin binding domain (HBD) of Fn decreases 125I-Fn binding to  M. tuberculosis; whereas MAbs specific to either the cell binding domain (CBD) or the gelatin binding domain (GBD) have no effect on Fn binding to  M. tuberculosis.	bind
49272	3	11076	7	10	NULL	NULL	NULL	Fn MAb	GP		does not affect			CBD		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_3_1287_s_5	11854212	A monoclonal antibody (MAb) specific to the heparin binding domain (HBD) of Fn decreases 125I-Fn binding to  M. tuberculosis; whereas MAbs specific to either the cell binding domain (CBD) or the gelatin binding domain (GBD) have no effect on Fn binding to  M. tuberculosis.	bind
49273	4	11076	7	10	NULL	NULL	NULL	Fn MAb	GP		does not affect			GBD		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_3_1287_s_5	11854212	A monoclonal antibody (MAb) specific to the heparin binding domain (HBD) of Fn decreases 125I-Fn binding to  M. tuberculosis; whereas MAbs specific to either the cell binding domain (CBD) or the gelatin binding domain (GBD) have no effect on Fn binding to  M. tuberculosis.	bind
49274	5	11076	7	10	NULL	NULL	NULL	MAb	GP		is					monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_3_1287_s_5	11854212	A monoclonal antibody (MAb) specific to the heparin binding domain (HBD) of Fn decreases 125I-Fn binding to  M. tuberculosis; whereas MAbs specific to either the cell binding domain (CBD) or the gelatin binding domain (GBD) have no effect on Fn binding to  M. tuberculosis.	bind
49275	6	11076	7	10	NULL	NULL	NULL	HBD	AminoAcid		is					heparin binding domain	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_3_1287_s_5	11854212	A monoclonal antibody (MAb) specific to the heparin binding domain (HBD) of Fn decreases 125I-Fn binding to  M. tuberculosis; whereas MAbs specific to either the cell binding domain (CBD) or the gelatin binding domain (GBD) have no effect on Fn binding to  M. tuberculosis.	bind
49276	7	11076	7	10	NULL	NULL	NULL	CBD	AminoAcid		is 					cell binding domain	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_3_1287_s_5	11854212	A monoclonal antibody (MAb) specific to the heparin binding domain (HBD) of Fn decreases 125I-Fn binding to  M. tuberculosis; whereas MAbs specific to either the cell binding domain (CBD) or the gelatin binding domain (GBD) have no effect on Fn binding to  M. tuberculosis.	bind
49277	8	11076	7	10	NULL	NULL	NULL	GBD	AminoAcid		is					gelatin binding domain	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_3_1287_s_5	11854212	A monoclonal antibody (MAb) specific to the heparin binding domain (HBD) of Fn decreases 125I-Fn binding to  M. tuberculosis; whereas MAbs specific to either the cell binding domain (CBD) or the gelatin binding domain (GBD) have no effect on Fn binding to  M. tuberculosis.	bind
42627	1	11077	6	10	NULL	NULL	NULL	MV	Organism		is					measles virus	Organism				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-virol_67_10_8371352_s_2	8371352	A monoclonal antibody (MCI20.6) which inhibited measles virus (MV) binding  to host cells was previously used to characterize a 57- to 67-kDa cell  surface glycoprotein as a potential MV receptor.	bind
42628	2	11077	6	10	NULL	NULL	NULL	MV	Organism		bind					host cells	Cell				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-virol_67_10_8371352_s_2	8371352	A monoclonal antibody (MCI20.6) which inhibited measles virus (MV) binding  to host cells was previously used to characterize a 57- to 67-kDa cell  surface glycoprotein as a potential MV receptor.	bind
42629	3	11077	6	10	NULL	NULL	NULL	MCI20.6	GP		is a type of					monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-virol_67_10_8371352_s_2	8371352	A monoclonal antibody (MCI20.6) which inhibited measles virus (MV) binding  to host cells was previously used to characterize a 57- to 67-kDa cell  surface glycoprotein as a potential MV receptor.	bind
42630	4	11077	6	10	NULL	NULL	NULL	MCI20.6	GP		inhibits					statement 2	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-virol_67_10_8371352_s_2	8371352	A monoclonal antibody (MCI20.6) which inhibited measles virus (MV) binding  to host cells was previously used to characterize a 57- to 67-kDa cell  surface glycoprotein as a potential MV receptor.	bind
49278	1	11077	7	10	NULL	NULL	NULL	MV	Organism		bind					host cells	Cell				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-virol_67_10_8371352_s_2	8371352	A monoclonal antibody (MCI20.6) which inhibited measles virus (MV) binding  to host cells was previously used to characterize a 57- to 67-kDa cell  surface glycoprotein as a potential MV receptor.	bind
49279	2	11077	7	10	NULL	NULL	NULL	MCI20.6	GP		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-virol_67_10_8371352_s_2	8371352	A monoclonal antibody (MCI20.6) which inhibited measles virus (MV) binding  to host cells was previously used to characterize a 57- to 67-kDa cell  surface glycoprotein as a potential MV receptor.	bind
49281	4	11077	7	10	NULL	NULL	NULL	MCI20.6	GP		is a type of					monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-virol_67_10_8371352_s_2	8371352	A monoclonal antibody (MCI20.6) which inhibited measles virus (MV) binding  to host cells was previously used to characterize a 57- to 67-kDa cell  surface glycoprotein as a potential MV receptor.	bind
49282	3	11077	7	10	NULL	NULL	NULL	MV	Organism		is 					measles virus	Organism				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-virol_67_10_8371352_s_2	8371352	A monoclonal antibody (MCI20.6) which inhibited measles virus (MV) binding  to host cells was previously used to characterize a 57- to 67-kDa cell  surface glycoprotein as a potential MV receptor.	bind
42631	1	11078	6	10	NULL	NULL	NULL	DR5	GP		is 					death receptor 5	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_clin-cancer-res_9_10-pt-1_14506165_s_3	14506165	A monoclonal antibody (TRA-8) has been developed that binds to  death receptor 5 (DR5), one of two death receptors bound by tumor necrosis  factor-related apoptosis-inducing ligand.	bind
42632	2	11078	6	10	NULL	NULL	NULL	TRA-8	GP		is a type of					monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_clin-cancer-res_9_10-pt-1_14506165_s_3	14506165	A monoclonal antibody (TRA-8) has been developed that binds to  death receptor 5 (DR5), one of two death receptors bound by tumor necrosis  factor-related apoptosis-inducing ligand.	bind
42633	3	11078	6	10	NULL	NULL	NULL	TR-8	GP		bind					DR-5	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_clin-cancer-res_9_10-pt-1_14506165_s_3	14506165	A monoclonal antibody (TRA-8) has been developed that binds to  death receptor 5 (DR5), one of two death receptors bound by tumor necrosis  factor-related apoptosis-inducing ligand.	bind
42634	4	11078	6	10	NULL	NULL	NULL	DR-5	GP		bind					tumor necrosis factor-related apoptosis-inducing ligand	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_clin-cancer-res_9_10-pt-1_14506165_s_3	14506165	A monoclonal antibody (TRA-8) has been developed that binds to  death receptor 5 (DR5), one of two death receptors bound by tumor necrosis  factor-related apoptosis-inducing ligand.	bind
49283	1	11078	7	10	NULL	NULL	NULL	TRA-8	GP		bind					DR5	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_clin-cancer-res_9_10-pt-1_14506165_s_3	14506165	A monoclonal antibody (TRA-8) has been developed that binds to  death receptor 5 (DR5), one of two death receptors bound by tumor necrosis  factor-related apoptosis-inducing ligand.	bind
49284	2	11078	7	10	NULL	NULL	NULL	TRA-8	GP		is a type of					monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_clin-cancer-res_9_10-pt-1_14506165_s_3	14506165	A monoclonal antibody (TRA-8) has been developed that binds to  death receptor 5 (DR5), one of two death receptors bound by tumor necrosis  factor-related apoptosis-inducing ligand.	bind
49285	3	11078	7	10	NULL	NULL	NULL	DR5	GP		is a type of					death receptor	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_clin-cancer-res_9_10-pt-1_14506165_s_3	14506165	A monoclonal antibody (TRA-8) has been developed that binds to  death receptor 5 (DR5), one of two death receptors bound by tumor necrosis  factor-related apoptosis-inducing ligand.	bind
49286	4	11078	7	10	NULL	NULL	NULL	tumor necrosis factor-related apoptosis-inducing ligand	GP		bind					DR5	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_clin-cancer-res_9_10-pt-1_14506165_s_3	14506165	A monoclonal antibody (TRA-8) has been developed that binds to  death receptor 5 (DR5), one of two death receptors bound by tumor necrosis  factor-related apoptosis-inducing ligand.	bind
42884	1	11080	6	10	NULL	NULL	NULL	CD24 	GP	substrate coated	elicits					neurite outgrowth	Process	negative influence on			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_24_21656_s_135	11283023	A monoclonal antibody against CD24 and polyclonal antibodies against L1 were able to reduce or inhibit the negative influences on neurite outgrowth elicited by substrate-coated CD24 but not on poly-L-lysine (Fig.  3 A, compare CD24 + anti-CD24 and CD24 + anti-L1 with CD24 and PLL), whereas nonimmune IgG control antibodies had no effect (Fig.  3 A, compare CD24 + IgG with CD24), indicating that the L1 antibody binds to L1 at the cell surface of dorsal root ganglion neurons and masks it for binding to CD24 in trans-interaction.	bind
42885	2	11080	6	10	NULL	NULL	NULL	L1 antibody	GP		bind					L1	GP				NULL	cell surface of dorsal root ganglion neurons	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_24_21656_s_135	11283023	A monoclonal antibody against CD24 and polyclonal antibodies against L1 were able to reduce or inhibit the negative influences on neurite outgrowth elicited by substrate-coated CD24 but not on poly-L-lysine (Fig.  3 A, compare CD24 + anti-CD24 and CD24 + anti-L1 with CD24 and PLL), whereas nonimmune IgG control antibodies had no effect (Fig.  3 A, compare CD24 + IgG with CD24), indicating that the L1 antibody binds to L1 at the cell surface of dorsal root ganglion neurons and masks it for binding to CD24 in trans-interaction.	bind
42886	3	11080	6	10	NULL	NULL	NULL	monoclonal antibody	GP		against					CD24	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_24_21656_s_135	11283023	A monoclonal antibody against CD24 and polyclonal antibodies against L1 were able to reduce or inhibit the negative influences on neurite outgrowth elicited by substrate-coated CD24 but not on poly-L-lysine (Fig.  3 A, compare CD24 + anti-CD24 and CD24 + anti-L1 with CD24 and PLL), whereas nonimmune IgG control antibodies had no effect (Fig.  3 A, compare CD24 + IgG with CD24), indicating that the L1 antibody binds to L1 at the cell surface of dorsal root ganglion neurons and masks it for binding to CD24 in trans-interaction.	bind
42887	4	11080	6	10	NULL	NULL	NULL	statement 3	Process		reduce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_24_21656_s_135	11283023	A monoclonal antibody against CD24 and polyclonal antibodies against L1 were able to reduce or inhibit the negative influences on neurite outgrowth elicited by substrate-coated CD24 but not on poly-L-lysine (Fig.  3 A, compare CD24 + anti-CD24 and CD24 + anti-L1 with CD24 and PLL), whereas nonimmune IgG control antibodies had no effect (Fig.  3 A, compare CD24 + IgG with CD24), indicating that the L1 antibody binds to L1 at the cell surface of dorsal root ganglion neurons and masks it for binding to CD24 in trans-interaction.	bind
42888	5	11080	6	10	NULL	NULL	NULL	Polyclonal antibodies	GP		against					L1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_24_21656_s_135	11283023	A monoclonal antibody against CD24 and polyclonal antibodies against L1 were able to reduce or inhibit the negative influences on neurite outgrowth elicited by substrate-coated CD24 but not on poly-L-lysine (Fig.  3 A, compare CD24 + anti-CD24 and CD24 + anti-L1 with CD24 and PLL), whereas nonimmune IgG control antibodies had no effect (Fig.  3 A, compare CD24 + IgG with CD24), indicating that the L1 antibody binds to L1 at the cell surface of dorsal root ganglion neurons and masks it for binding to CD24 in trans-interaction.	bind
42889	6	11080	6	10	NULL	NULL	NULL	statement 5	Process		reduce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_24_21656_s_135	11283023	A monoclonal antibody against CD24 and polyclonal antibodies against L1 were able to reduce or inhibit the negative influences on neurite outgrowth elicited by substrate-coated CD24 but not on poly-L-lysine (Fig.  3 A, compare CD24 + anti-CD24 and CD24 + anti-L1 with CD24 and PLL), whereas nonimmune IgG control antibodies had no effect (Fig.  3 A, compare CD24 + IgG with CD24), indicating that the L1 antibody binds to L1 at the cell surface of dorsal root ganglion neurons and masks it for binding to CD24 in trans-interaction.	bind
42890	7	11080	6	10	NULL	NULL	NULL	L1	GP		bind					CD24	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_24_21656_s_135	11283023	A monoclonal antibody against CD24 and polyclonal antibodies against L1 were able to reduce or inhibit the negative influences on neurite outgrowth elicited by substrate-coated CD24 but not on poly-L-lysine (Fig.  3 A, compare CD24 + anti-CD24 and CD24 + anti-L1 with CD24 and PLL), whereas nonimmune IgG control antibodies had no effect (Fig.  3 A, compare CD24 + IgG with CD24), indicating that the L1 antibody binds to L1 at the cell surface of dorsal root ganglion neurons and masks it for binding to CD24 in trans-interaction.	bind
42891	8	11080	6	10	NULL	NULL	NULL	statement 2	Process		masks					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_24_21656_s_135	11283023	A monoclonal antibody against CD24 and polyclonal antibodies against L1 were able to reduce or inhibit the negative influences on neurite outgrowth elicited by substrate-coated CD24 but not on poly-L-lysine (Fig.  3 A, compare CD24 + anti-CD24 and CD24 + anti-L1 with CD24 and PLL), whereas nonimmune IgG control antibodies had no effect (Fig.  3 A, compare CD24 + IgG with CD24), indicating that the L1 antibody binds to L1 at the cell surface of dorsal root ganglion neurons and masks it for binding to CD24 in trans-interaction.	bind
49287	1	11080	7	10	NULL	NULL	NULL	L1 antibody	GP		bind					L1	GP				NULL	cell surface of dorsal root ganglion neurons	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_24_21656_s_135	11283023	A monoclonal antibody against CD24 and polyclonal antibodies against L1 were able to reduce or inhibit the negative influences on neurite outgrowth elicited by substrate-coated CD24 but not on poly-L-lysine (Fig.  3 A, compare CD24 + anti-CD24 and CD24 + anti-L1 with CD24 and PLL), whereas nonimmune IgG control antibodies had no effect (Fig.  3 A, compare CD24 + IgG with CD24), indicating that the L1 antibody binds to L1 at the cell surface of dorsal root ganglion neurons and masks it for binding to CD24 in trans-interaction.	bind
49288	2	11080	7	10	NULL	NULL	NULL	L1	GP		bind					CD24	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_24_21656_s_135	11283023	A monoclonal antibody against CD24 and polyclonal antibodies against L1 were able to reduce or inhibit the negative influences on neurite outgrowth elicited by substrate-coated CD24 but not on poly-L-lysine (Fig.  3 A, compare CD24 + anti-CD24 and CD24 + anti-L1 with CD24 and PLL), whereas nonimmune IgG control antibodies had no effect (Fig.  3 A, compare CD24 + IgG with CD24), indicating that the L1 antibody binds to L1 at the cell surface of dorsal root ganglion neurons and masks it for binding to CD24 in trans-interaction.	bind
49289	3	11080	7	10	NULL	NULL	NULL	statement 1	Process		masks					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_24_21656_s_135	11283023	A monoclonal antibody against CD24 and polyclonal antibodies against L1 were able to reduce or inhibit the negative influences on neurite outgrowth elicited by substrate-coated CD24 but not on poly-L-lysine (Fig.  3 A, compare CD24 + anti-CD24 and CD24 + anti-L1 with CD24 and PLL), whereas nonimmune IgG control antibodies had no effect (Fig.  3 A, compare CD24 + IgG with CD24), indicating that the L1 antibody binds to L1 at the cell surface of dorsal root ganglion neurons and masks it for binding to CD24 in trans-interaction.	bind
49290	4	11080	7	10	NULL	NULL	NULL	statement 2	Process		occurs in					trans-interaction	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_24_21656_s_135	11283023	A monoclonal antibody against CD24 and polyclonal antibodies against L1 were able to reduce or inhibit the negative influences on neurite outgrowth elicited by substrate-coated CD24 but not on poly-L-lysine (Fig.  3 A, compare CD24 + anti-CD24 and CD24 + anti-L1 with CD24 and PLL), whereas nonimmune IgG control antibodies had no effect (Fig.  3 A, compare CD24 + IgG with CD24), indicating that the L1 antibody binds to L1 at the cell surface of dorsal root ganglion neurons and masks it for binding to CD24 in trans-interaction.	bind
42892	1	11081	6	10	NULL	NULL	NULL	monoclonal antibody	GP		is directed against					GAF 	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_22_3_469_s_6	12554648	A monoclonal antibody directed against GAF A blocked cGMP binding, prevented  PDE5 activation and decreased basal activity, revealing that PDE5 in its non-activated  state has low intrinsic catalytic activity.	bind
42893	2	11081	6	10	NULL	NULL	NULL	statement 1	Process		blocks					cGMP	Chemical	binding of 			NULL		NULL	NULL	NULL	NULL	gw70_embo_22_3_469_s_6	12554648	A monoclonal antibody directed against GAF A blocked cGMP binding, prevented  PDE5 activation and decreased basal activity, revealing that PDE5 in its non-activated  state has low intrinsic catalytic activity.	bind
42894	3	11081	6	10	NULL	NULL	NULL	statement 1	Process		prevents					PDE5	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_embo_22_3_469_s_6	12554648	A monoclonal antibody directed against GAF A blocked cGMP binding, prevented  PDE5 activation and decreased basal activity, revealing that PDE5 in its non-activated  state has low intrinsic catalytic activity.	bind
42895	4	11081	6	10	NULL	NULL	NULL	PDE5	GP	non-activated	possess					catalytic activity	Process	low;; intrinsic			NULL		NULL	NULL	NULL	NULL	gw70_embo_22_3_469_s_6	12554648	A monoclonal antibody directed against GAF A blocked cGMP binding, prevented  PDE5 activation and decreased basal activity, revealing that PDE5 in its non-activated  state has low intrinsic catalytic activity.	bind
49291	1	11081	7	10	NULL	NULL	NULL	GAF A monoclonal antibody	GP		blocks					cGMP	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw70_embo_22_3_469_s_6	12554648	A monoclonal antibody directed against GAF A blocked cGMP binding, prevented  PDE5 activation and decreased basal activity, revealing that PDE5 in its non-activated  state has low intrinsic catalytic activity.	bind
49292	2	11081	7	10	NULL	NULL	NULL	GAF A monoclonal antibody	GP		prevents					PDE5	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_embo_22_3_469_s_6	12554648	A monoclonal antibody directed against GAF A blocked cGMP binding, prevented  PDE5 activation and decreased basal activity, revealing that PDE5 in its non-activated  state has low intrinsic catalytic activity.	bind
49294	3	11081	7	10	NULL	NULL	NULL	PDE5	GP	 non-activated	possess 					catalytic activity	Process	low;;intrinsic 			NULL		NULL	NULL	NULL	NULL	gw70_embo_22_3_469_s_6	12554648	A monoclonal antibody directed against GAF A blocked cGMP binding, prevented  PDE5 activation and decreased basal activity, revealing that PDE5 in its non-activated  state has low intrinsic catalytic activity.	bind
42670	1	11083	6	10	NULL	NULL	NULL	uPA	GP	human	bind					uPAR	GP	human			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_am-j-physiol_277_3-pt-1_10484465_s_6	10484465	A monoclonal antibody that blocks  the binding of human uPA to human uPAR suppressed fibrin degradation by  human cells expressing human uPA but not murine uPA.	bind
42671	2	11083	6	10	NULL	NULL	NULL	cells	Cell	human	express					uPA	GP	human			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_am-j-physiol_277_3-pt-1_10484465_s_6	10484465	A monoclonal antibody that blocks  the binding of human uPA to human uPAR suppressed fibrin degradation by  human cells expressing human uPA but not murine uPA.	bind
42672	3	11083	6	10	NULL	NULL	NULL	statement 2	Process		degrades					fibrin	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_am-j-physiol_277_3-pt-1_10484465_s_6	10484465	A monoclonal antibody that blocks  the binding of human uPA to human uPAR suppressed fibrin degradation by  human cells expressing human uPA but not murine uPA.	bind
57867	4	11083	6	10	NULL	NULL	NULL	cells	Cell	human	express					uPA	GP	murine			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_am-j-physiol_277_3-pt-1_10484465_s_6	10484465	A monoclonal antibody that blocks  the binding of human uPA to human uPAR suppressed fibrin degradation by  human cells expressing human uPA but not murine uPA.	bind
57868	5	11083	6	10	NULL	NULL	NULL	statement 4	Process		degrades					fibrin	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_am-j-physiol_277_3-pt-1_10484465_s_6	10484465	A monoclonal antibody that blocks  the binding of human uPA to human uPAR suppressed fibrin degradation by  human cells expressing human uPA but not murine uPA.	bind
57869	6	11083	6	10	NULL	NULL	NULL	monoclonal antibody	GP		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_am-j-physiol_277_3-pt-1_10484465_s_6	10484465	A monoclonal antibody that blocks  the binding of human uPA to human uPAR suppressed fibrin degradation by  human cells expressing human uPA but not murine uPA.	bind
57870	7	11083	6	10	NULL	NULL	NULL	monoclonal antibody	GP		supress					statement 3	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_am-j-physiol_277_3-pt-1_10484465_s_6	10484465	A monoclonal antibody that blocks  the binding of human uPA to human uPAR suppressed fibrin degradation by  human cells expressing human uPA but not murine uPA.	bind
57871	8	11083	6	10	NULL	NULL	NULL	monoclonal antibody	GP		does not supress					statement 5	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_am-j-physiol_277_3-pt-1_10484465_s_6	10484465	A monoclonal antibody that blocks  the binding of human uPA to human uPAR suppressed fibrin degradation by  human cells expressing human uPA but not murine uPA.	bind
49295	1	11083	7	10	NULL	NULL	NULL	 uPA 	GP	human	bind					uPAR	GP	human			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_am-j-physiol_277_3-pt-1_10484465_s_6	10484465	A monoclonal antibody that blocks  the binding of human uPA to human uPAR suppressed fibrin degradation by  human cells expressing human uPA but not murine uPA.	bind
49296	2	11083	7	10	NULL	NULL	NULL	monoclonal antibody	GP		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_am-j-physiol_277_3-pt-1_10484465_s_6	10484465	A monoclonal antibody that blocks  the binding of human uPA to human uPAR suppressed fibrin degradation by  human cells expressing human uPA but not murine uPA.	bind
49297	3	11083	7	10	NULL	NULL	NULL	cells	Cell	human	express					uPA	GP	human			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_am-j-physiol_277_3-pt-1_10484465_s_6	10484465	A monoclonal antibody that blocks  the binding of human uPA to human uPAR suppressed fibrin degradation by  human cells expressing human uPA but not murine uPA.	bind
49298	4	11083	7	10	NULL	NULL	NULL	cells	Cell	human	express					uPA	GP	murine			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_am-j-physiol_277_3-pt-1_10484465_s_6	10484465	A monoclonal antibody that blocks  the binding of human uPA to human uPAR suppressed fibrin degradation by  human cells expressing human uPA but not murine uPA.	bind
49299	5	11083	7	10	NULL	NULL	NULL	statement 3	Process		degrades					fibrin	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_am-j-physiol_277_3-pt-1_10484465_s_6	10484465	A monoclonal antibody that blocks  the binding of human uPA to human uPAR suppressed fibrin degradation by  human cells expressing human uPA but not murine uPA.	bind
49300	6	11083	7	10	NULL	NULL	NULL	statement 4	Process		degrades					fibrin	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_am-j-physiol_277_3-pt-1_10484465_s_6	10484465	A monoclonal antibody that blocks  the binding of human uPA to human uPAR suppressed fibrin degradation by  human cells expressing human uPA but not murine uPA.	bind
49301	7	11083	7	10	NULL	NULL	NULL	monoclonal antibody	GP		suppress					statement 5	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_am-j-physiol_277_3-pt-1_10484465_s_6	10484465	A monoclonal antibody that blocks  the binding of human uPA to human uPAR suppressed fibrin degradation by  human cells expressing human uPA but not murine uPA.	bind
49302	8	11083	7	10	NULL	NULL	NULL	monoclonal antibody	GP		does not suppress					statement 6	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_am-j-physiol_277_3-pt-1_10484465_s_6	10484465	A monoclonal antibody that blocks  the binding of human uPA to human uPAR suppressed fibrin degradation by  human cells expressing human uPA but not murine uPA.	bind
42673	1	11084	6	10	NULL	NULL	NULL	MCP-1	GP		bind					CCR2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_9_858_s_198	15514167	A monoclonal antibody that blocks the binding of MCP-1 to CCR2 is being used in phase II trials for rheumatoid arthritis, and CCR5 antagonists that block HIV entry into cells are being used in advanced clinical trials as adjuvant treatments for AIDS.	bind
42681	2	11084	6	10	NULL	NULL	NULL	HIV	Organism		enters into					cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_9_858_s_198	15514167	A monoclonal antibody that blocks the binding of MCP-1 to CCR2 is being used in phase II trials for rheumatoid arthritis, and CCR5 antagonists that block HIV entry into cells are being used in advanced clinical trials as adjuvant treatments for AIDS.	bind
42682	3	11084	6	10	NULL	NULL	NULL	CCR5 antagonist	Chemical		blocks					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_9_858_s_198	15514167	A monoclonal antibody that blocks the binding of MCP-1 to CCR2 is being used in phase II trials for rheumatoid arthritis, and CCR5 antagonists that block HIV entry into cells are being used in advanced clinical trials as adjuvant treatments for AIDS.	bind
49303	1	11084	7	10	NULL	NULL	NULL	MCP-1 	GP		bind					CCR2	GP				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_9_858_s_198	15514167	A monoclonal antibody that blocks the binding of MCP-1 to CCR2 is being used in phase II trials for rheumatoid arthritis, and CCR5 antagonists that block HIV entry into cells are being used in advanced clinical trials as adjuvant treatments for AIDS.	bind
49304	2	11084	7	10	NULL	NULL	NULL	monoclonal antibody	GP		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_9_858_s_198	15514167	A monoclonal antibody that blocks the binding of MCP-1 to CCR2 is being used in phase II trials for rheumatoid arthritis, and CCR5 antagonists that block HIV entry into cells are being used in advanced clinical trials as adjuvant treatments for AIDS.	bind
49305	3	11084	7	10	NULL	NULL	NULL	HIV	Organism		enter into					cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_9_858_s_198	15514167	A monoclonal antibody that blocks the binding of MCP-1 to CCR2 is being used in phase II trials for rheumatoid arthritis, and CCR5 antagonists that block HIV entry into cells are being used in advanced clinical trials as adjuvant treatments for AIDS.	bind
49306	4	11084	7	10	NULL	NULL	NULL	CCR5 antagonists	Chemical		block					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_9_858_s_198	15514167	A monoclonal antibody that blocks the binding of MCP-1 to CCR2 is being used in phase II trials for rheumatoid arthritis, and CCR5 antagonists that block HIV entry into cells are being used in advanced clinical trials as adjuvant treatments for AIDS.	bind
42683	1	11086	6	10	NULL	NULL	NULL	sperm	Cell	human	bind					oolemma	CellComponent	hamster			NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_67_3_795_s_308	12193387	A monoclonal antibody to human SP-10 inhibits in vitro the binding of human sperm to hamster oolemma but not to human zona pellucida.	bind
42684	2	11086	6	10	NULL	NULL	NULL	sperm	Cell	human	bind					zona pellucida	CellComponent	human			NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_67_3_795_s_308	12193387	A monoclonal antibody to human SP-10 inhibits in vitro the binding of human sperm to hamster oolemma but not to human zona pellucida.	bind
50281	3	11086	6	10	NULL	NULL	NULL	monoclonal antibody to SP-10	GP	human	inhibit					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_biolreprod_67_3_795_s_308	12193387	A monoclonal antibody to human SP-10 inhibits in vitro the binding of human sperm to hamster oolemma but not to human zona pellucida.	bind
50282	4	11086	6	10	NULL	NULL	NULL	monoclonal antibody to SP-10	GP	human	does not inhibit					statement 2	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_biolreprod_67_3_795_s_308	12193387	A monoclonal antibody to human SP-10 inhibits in vitro the binding of human sperm to hamster oolemma but not to human zona pellucida.	bind
49309	1	11086	7	10	NULL	NULL	NULL	sperm 	Cell	human	bind					oolemma	CellComponent	hamster			NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_67_3_795_s_308	12193387	A monoclonal antibody to human SP-10 inhibits in vitro the binding of human sperm to hamster oolemma but not to human zona pellucida.	bind
49310	2	11086	7	10	NULL	NULL	NULL	sperm	Cell	human	bind					zona pellucida	CellComponent	human			NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_67_3_795_s_308	12193387	A monoclonal antibody to human SP-10 inhibits in vitro the binding of human sperm to hamster oolemma but not to human zona pellucida.	bind
49311	3	11086	7	10	NULL	NULL	NULL	monoclonal antibody to SP-10	GP	human	inhibit					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_biolreprod_67_3_795_s_308	12193387	A monoclonal antibody to human SP-10 inhibits in vitro the binding of human sperm to hamster oolemma but not to human zona pellucida.	bind
49312	4	11086	7	10	NULL	NULL	NULL	monoclonal antibody to SP-10	GP	human	does not inhibit					statement 2	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_biolreprod_67_3_795_s_308	12193387	A monoclonal antibody to human SP-10 inhibits in vitro the binding of human sperm to hamster oolemma but not to human zona pellucida.	bind
42686	1	11088	6	10	NULL	NULL	NULL	CDK2	GP		bind					GST:SNR1	GP				NULL		NULL	NULL	NULL	NULL	gw70_genetics_168_1_199_s_209	15454538	A monoclonal antibody to the MYC epitope identified CDK2 bound to the GST:SNR1 fusion, but not GST alone.	bind
57872	2	11088	6	10	NULL	NULL	NULL	GST:SNR1	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_genetics_168_1_199_s_209	15454538	A monoclonal antibody to the MYC epitope identified CDK2 bound to the GST:SNR1 fusion, but not GST alone.	bind
49314	1	11088	7	10	NULL	NULL	NULL	 CDK2	GP		bind					GST:SNR1	GP				NULL		NULL	NULL	NULL	NULL	gw70_genetics_168_1_199_s_209	15454538	A monoclonal antibody to the MYC epitope identified CDK2 bound to the GST:SNR1 fusion, but not GST alone.	bind
57873	2	11088	7	10	NULL	NULL	NULL	GST:SNR1	GP		is a type of					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_genetics_168_1_199_s_209	15454538	A monoclonal antibody to the MYC epitope identified CDK2 bound to the GST:SNR1 fusion, but not GST alone.	bind
42687	1	11089	6	10	NULL	NULL	NULL	LPS	Chemical		bind					CD14	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_11_5357_s_95	9784544	A monoclonal antibody, 26iC (10 mug/ml), which recognizes CD14 but does not block LPS binding to CD14, was used as a control.	bind
42688	2	11089	6	10	NULL	NULL	NULL	26iC	GP		is a type of					monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_11_5357_s_95	9784544	A monoclonal antibody, 26iC (10 mug/ml), which recognizes CD14 but does not block LPS binding to CD14, was used as a control.	bind
42689	3	11089	6	10	NULL	NULL	NULL	26iC	GP		recognizes					CD14	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_11_5357_s_95	9784544	A monoclonal antibody, 26iC (10 mug/ml), which recognizes CD14 but does not block LPS binding to CD14, was used as a control.	bind
42690	4	11089	6	10	NULL	NULL	NULL	26iC	GP		does not block					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_11_5357_s_95	9784544	A monoclonal antibody, 26iC (10 mug/ml), which recognizes CD14 but does not block LPS binding to CD14, was used as a control.	bind
49317	1	11089	7	10	NULL	NULL	NULL	LPS	Chemical		bind					CD14	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_11_5357_s_95	9784544	A monoclonal antibody, 26iC (10 mug/ml), which recognizes CD14 but does not block LPS binding to CD14, was used as a control.	bind
49318	2	11089	7	10	NULL	NULL	NULL	 26iC	GP		recognizes					CD14	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_11_5357_s_95	9784544	A monoclonal antibody, 26iC (10 mug/ml), which recognizes CD14 but does not block LPS binding to CD14, was used as a control.	bind
49319	3	11089	7	10	NULL	NULL	NULL	 26iC	GP		does not block					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_11_5357_s_95	9784544	A monoclonal antibody, 26iC (10 mug/ml), which recognizes CD14 but does not block LPS binding to CD14, was used as a control.	bind
49320	4	11089	7	10	NULL	NULL	NULL	 26iC	GP		is a type of					monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_11_5357_s_95	9784544	A monoclonal antibody, 26iC (10 mug/ml), which recognizes CD14 but does not block LPS binding to CD14, was used as a control.	bind
42691	1	11090	6	10	NULL	NULL	NULL	APC	GP		bind					EPCR	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_j-invest-dermatol_125_6_16354200_s_8	16354200	A monoclonal antibody, RCR252, which blocks APC binding  to EPCR, or a blocking antibody to PAR-1, abolished APC's effects on keratinocytes.	bind
42692	2	11090	6	10	NULL	NULL	NULL	RCR252	GP		is a type of					monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_j-invest-dermatol_125_6_16354200_s_8	16354200	A monoclonal antibody, RCR252, which blocks APC binding  to EPCR, or a blocking antibody to PAR-1, abolished APC's effects on keratinocytes.	bind
42693	3	11090	6	10	NULL	NULL	NULL	RCR252	GP		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_j-invest-dermatol_125_6_16354200_s_8	16354200	A monoclonal antibody, RCR252, which blocks APC binding  to EPCR, or a blocking antibody to PAR-1, abolished APC's effects on keratinocytes.	bind
42694	4	11090	6	10	NULL	NULL	NULL	APC	GP		effects					keratinocytes	Cell				NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_j-invest-dermatol_125_6_16354200_s_8	16354200	A monoclonal antibody, RCR252, which blocks APC binding  to EPCR, or a blocking antibody to PAR-1, abolished APC's effects on keratinocytes.	bind
42695	5	11090	6	10	NULL	NULL	NULL	blocking antibody to PAR-1	GP		abolishes					statement 4	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_j-invest-dermatol_125_6_16354200_s_8	16354200	A monoclonal antibody, RCR252, which blocks APC binding  to EPCR, or a blocking antibody to PAR-1, abolished APC's effects on keratinocytes.	bind
49321	1	11090	7	10	NULL	NULL	NULL	APC	GP		bind					EPCR	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_j-invest-dermatol_125_6_16354200_s_8	16354200	A monoclonal antibody, RCR252, which blocks APC binding  to EPCR, or a blocking antibody to PAR-1, abolished APC's effects on keratinocytes.	bind
49322	2	11090	7	10	NULL	NULL	NULL	RCR252	GP		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_j-invest-dermatol_125_6_16354200_s_8	16354200	A monoclonal antibody, RCR252, which blocks APC binding  to EPCR, or a blocking antibody to PAR-1, abolished APC's effects on keratinocytes.	bind
49323	3	11090	7	10	NULL	NULL	NULL	PAR-1 blocking antibody	GP		abolishes					APCs	GP	effect of			NULL	keratinocytes	NULL	NULL	NULL	NULL	abs-batch0550-0559_j-invest-dermatol_125_6_16354200_s_8	16354200	A monoclonal antibody, RCR252, which blocks APC binding  to EPCR, or a blocking antibody to PAR-1, abolished APC's effects on keratinocytes.	bind
49324	4	11090	7	10	NULL	NULL	NULL	RCR252	GP		is a type of					monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_j-invest-dermatol_125_6_16354200_s_8	16354200	A monoclonal antibody, RCR252, which blocks APC binding  to EPCR, or a blocking antibody to PAR-1, abolished APC's effects on keratinocytes.	bind
42696	1	11091	6	10	NULL	NULL	NULL	TRA-8	GP		is a type of					monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_cancer-gene-ther_13_2_16082379_s_4	16082379	A monoclonal antibody, TRA-8, specifically binds  to death receptor 5, one of two death receptors bound by tumor necrosis  factor-related apoptosis-inducing ligand (TRAIL).	bind
42697	2	11091	6	10	NULL	NULL	NULL	TRA-8	GP		bind		specifically			death receptor 5	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_cancer-gene-ther_13_2_16082379_s_4	16082379	A monoclonal antibody, TRA-8, specifically binds  to death receptor 5, one of two death receptors bound by tumor necrosis  factor-related apoptosis-inducing ligand (TRAIL).	bind
42698	3	11091	6	10	NULL	NULL	NULL	death receptor 5	GP		is a type of					death receptor	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_cancer-gene-ther_13_2_16082379_s_4	16082379	A monoclonal antibody, TRA-8, specifically binds  to death receptor 5, one of two death receptors bound by tumor necrosis  factor-related apoptosis-inducing ligand (TRAIL).	bind
42699	4	11091	6	10	NULL	NULL	NULL	death receptor 5	GP		bind					TRAIL	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_cancer-gene-ther_13_2_16082379_s_4	16082379	A monoclonal antibody, TRA-8, specifically binds  to death receptor 5, one of two death receptors bound by tumor necrosis  factor-related apoptosis-inducing ligand (TRAIL).	bind
42700	5	11091	6	10	NULL	NULL	NULL	TRAIL	GP		is					tumor necrosis factor-related apoptosis-inducing ligand	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_cancer-gene-ther_13_2_16082379_s_4	16082379	A monoclonal antibody, TRA-8, specifically binds  to death receptor 5, one of two death receptors bound by tumor necrosis  factor-related apoptosis-inducing ligand (TRAIL).	bind
49325	1	11091	7	10	NULL	NULL	NULL	TRA-8	GP		bind		specifically			death receptor 5	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_cancer-gene-ther_13_2_16082379_s_4	16082379	A monoclonal antibody, TRA-8, specifically binds  to death receptor 5, one of two death receptors bound by tumor necrosis  factor-related apoptosis-inducing ligand (TRAIL).	bind
49326	2	11091	7	10	NULL	NULL	NULL	TRAIL	GP		bind					death receptor 5	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_cancer-gene-ther_13_2_16082379_s_4	16082379	A monoclonal antibody, TRA-8, specifically binds  to death receptor 5, one of two death receptors bound by tumor necrosis  factor-related apoptosis-inducing ligand (TRAIL).	bind
49327	3	11091	7	10	NULL	NULL	NULL	TRA-8	GP		is a type of					monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_cancer-gene-ther_13_2_16082379_s_4	16082379	A monoclonal antibody, TRA-8, specifically binds  to death receptor 5, one of two death receptors bound by tumor necrosis  factor-related apoptosis-inducing ligand (TRAIL).	bind
49328	4	11091	7	10	NULL	NULL	NULL	TRAIL	GP		is					tumor necrosis factor-related apoptosis-inducing ligand	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_cancer-gene-ther_13_2_16082379_s_4	16082379	A monoclonal antibody, TRA-8, specifically binds  to death receptor 5, one of two death receptors bound by tumor necrosis  factor-related apoptosis-inducing ligand (TRAIL).	bind
50283	5	11091	7	10	NULL	NULL	NULL	TRA-8	GP		is a type of					monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_cancer-gene-ther_13_2_16082379_s_4	16082379	A monoclonal antibody, TRA-8, specifically binds  to death receptor 5, one of two death receptors bound by tumor necrosis  factor-related apoptosis-inducing ligand (TRAIL).	bind
42701	1	11092	6	10	NULL	NULL	NULL	nuclear proteins	GP	monocyte	bind					AP-2	GP	 Consensus Sequences			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_1_174_s_108	8995244	A Monocytic Nuclear Protein Binds to AP-2 Consensus Sequences	bind
49329	1	11092	7	10	NULL	NULL	NULL	Nuclear Protein	GP	Monocyte	bind					AP-2	GP	consensus sequence			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_1_174_s_108	8995244	A Monocytic Nuclear Protein Binds to AP-2 Consensus Sequences	bind
42702	1	11093	6	10	NULL	NULL	NULL	DnaA monomer	GP	E.coli	bind							stringent		DnaA box	NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiolrev_26_4_355_s_185	12413665	A monomer of  E. coli DnaA binds only to the stringent DnaA box.	bind
49339	1	11093	7	10	NULL	NULL	NULL	DnaA monomer	GP	E. coli	bind							stringent		DnaA box	NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiolrev_26_4_355_s_185	12413665	A monomer of  E. coli DnaA binds only to the stringent DnaA box.	bind
42780	1	11094	6	10	NULL	NULL	NULL	vancomysin monomer	GP		bind					disaccharide PG precursor	GP		dipeptidyl terminus		NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_26_5_511_s_376	12586393	A monomer of vancomycin binding the dipeptidyl  terminus of a disaccharide PG precursor (GlcNAc-MurNAc- -Ala- -Glu- -Lys- -Ala- -Ala) as it is delivered to the in vivo target site for transglycosylation by undecaprenyl  pyrophosphate (undecaprenol is depicted in red).	bind
42841	2	11094	6	10	NULL	NULL	NULL	disaccharide PG precursor	GP		is delivered to					target site					NULL	in vivo	NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_26_5_511_s_376	12586393	A monomer of vancomycin binding the dipeptidyl  terminus of a disaccharide PG precursor (GlcNAc-MurNAc- -Ala- -Glu- -Lys- -Ala- -Ala) as it is delivered to the in vivo target site for transglycosylation by undecaprenyl  pyrophosphate (undecaprenol is depicted in red).	bind
42842	3	11094	6	10	NULL	0	NULL	undecaprenyl pyrophosphate			catalyzes					disaccharide PG precursor		transglycosylation of 			NULL	in vivo	NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_26_5_511_s_376	12586393	A monomer of vancomycin binding the dipeptidyl  terminus of a disaccharide PG precursor (GlcNAc-MurNAc- -Ala- -Glu- -Lys- -Ala- -Ala) as it is delivered to the in vivo target site for transglycosylation by undecaprenyl  pyrophosphate (undecaprenol is depicted in red).	bind
42843	4	11094	6	10	NULL	NULL	NULL	statement 2	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_26_5_511_s_376	12586393	A monomer of vancomycin binding the dipeptidyl  terminus of a disaccharide PG precursor (GlcNAc-MurNAc- -Ala- -Glu- -Lys- -Ala- -Ala) as it is delivered to the in vivo target site for transglycosylation by undecaprenyl  pyrophosphate (undecaprenol is depicted in red).	bind
42844	5	11094	6	NULL	NULL	0	NULL	PG precursor	NULL		is	NULL				GlcNAc-MurNAc- -Ala- -Glu- -Lys- -Ala- -Ala	NULL				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_26_5_511_s_376	12586393	A monomer of vancomycin binding the dipeptidyl  terminus of a disaccharide PG precursor (GlcNAc-MurNAc- -Ala- -Glu- -Lys- -Ala- -Ala) as it is delivered to the in vivo target site for transglycosylation by undecaprenyl  pyrophosphate (undecaprenol is depicted in red).	bind
57874	6	11094	6	10	NULL	0	NULL	statement 1			leads to					statement 2					NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_26_5_511_s_376	12586393	A monomer of vancomycin binding the dipeptidyl  terminus of a disaccharide PG precursor (GlcNAc-MurNAc- -Ala- -Glu- -Lys- -Ala- -Ala) as it is delivered to the in vivo target site for transglycosylation by undecaprenyl  pyrophosphate (undecaprenol is depicted in red).	bind
49340	1	11094	7	NULL	NULL	0	NULL	vancomycin monomer	NULL		bind	NULL				disaccharide PG precursor	NULL		dipeptidyl terminus		NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_26_5_511_s_376	12586393	A monomer of vancomycin binding the dipeptidyl  terminus of a disaccharide PG precursor (GlcNAc-MurNAc- -Ala- -Glu- -Lys- -Ala- -Ala) as it is delivered to the in vivo target site for transglycosylation by undecaprenyl  pyrophosphate (undecaprenol is depicted in red).	bind
49341	2	11094	7	NULL	NULL	0	NULL	disaccharide PG precursor 	NULL		is	NULL				GlcNAc-MurNAc- -Ala- -Glu- -Lys- -Ala- -Ala	NULL				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_26_5_511_s_376	12586393	A monomer of vancomycin binding the dipeptidyl  terminus of a disaccharide PG precursor (GlcNAc-MurNAc- -Ala- -Glu- -Lys- -Ala- -Ala) as it is delivered to the in vivo target site for transglycosylation by undecaprenyl  pyrophosphate (undecaprenol is depicted in red).	bind
49342	3	11094	7	10	NULL	0	NULL	\tdisaccharide PG precursor			is delivered to					target site					NULL	in vivo	NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_26_5_511_s_376	12586393	A monomer of vancomycin binding the dipeptidyl  terminus of a disaccharide PG precursor (GlcNAc-MurNAc- -Ala- -Glu- -Lys- -Ala- -Ala) as it is delivered to the in vivo target site for transglycosylation by undecaprenyl  pyrophosphate (undecaprenol is depicted in red).	bind
49343	4	11094	7	10	NULL	0	NULL	undecaprenyl pyrophosphate			catalyzes					disaccharide PG precursor		transglycosylation of			NULL	in vivo	NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_26_5_511_s_376	12586393	A monomer of vancomycin binding the dipeptidyl  terminus of a disaccharide PG precursor (GlcNAc-MurNAc- -Ala- -Glu- -Lys- -Ala- -Ala) as it is delivered to the in vivo target site for transglycosylation by undecaprenyl  pyrophosphate (undecaprenol is depicted in red).	bind
49344	5	11094	7	10	NULL	0	NULL	statement 3			leads to					statement 4					NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_26_5_511_s_376	12586393	A monomer of vancomycin binding the dipeptidyl  terminus of a disaccharide PG precursor (GlcNAc-MurNAc- -Ala- -Glu- -Lys- -Ala- -Ala) as it is delivered to the in vivo target site for transglycosylation by undecaprenyl  pyrophosphate (undecaprenol is depicted in red).	bind
57875	6	11094	7	10	NULL	0	NULL	statement 1			leads to					statement 3					NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_26_5_511_s_376	12586393	A monomer of vancomycin binding the dipeptidyl  terminus of a disaccharide PG precursor (GlcNAc-MurNAc- -Ala- -Glu- -Lys- -Ala- -Ala) as it is delivered to the in vivo target site for transglycosylation by undecaprenyl  pyrophosphate (undecaprenol is depicted in red).	bind
42708	1	11096	6	10	NULL	NULL	NULL	Cu(I)	Chemical		bind					PDI	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_311_2_405_s_198	14592429	A mononuclear Cu(I) complex may either be linear (diagonal), trigonal, or tetragonal  coordinate; therefore in theory, the maximum Cu(I) bound to PDI is expected to be  2 mol/monomer.	bind
49345	1	11096	7	10	NULL	NULL	NULL	Cu(I)	Chemical		bind					PDI	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_311_2_405_s_198	14592429	A mononuclear Cu(I) complex may either be linear (diagonal), trigonal, or tetragonal  coordinate; therefore in theory, the maximum Cu(I) bound to PDI is expected to be  2 mol/monomer.	bind
42709	1	11097	6	10	NULL	NULL	NULL	ALG-2	GP		bind					annexin 7	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_22_20210_s_177	12601007	A more  recently identified ligand of annexin 11, namely the penta-EF-hand protein  ALG-2 (apoptosis-linked gene 2)  ( ) is expressed in the  nucleus ( ), though ALG-2  also binds annexin 7, peflin, and AIP1/Alix  ( ,   ).	bind
42710	2	11097	6	10	NULL	NULL	NULL	ALG-2	GP		bind					peflin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_22_20210_s_177	12601007	A more  recently identified ligand of annexin 11, namely the penta-EF-hand protein  ALG-2 (apoptosis-linked gene 2)  ( ) is expressed in the  nucleus ( ), though ALG-2  also binds annexin 7, peflin, and AIP1/Alix  ( ,   ).	bind
42711	3	11097	6	10	NULL	NULL	NULL	ALG-2	GP		bind					AIP1/Alix	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_22_20210_s_177	12601007	A more  recently identified ligand of annexin 11, namely the penta-EF-hand protein  ALG-2 (apoptosis-linked gene 2)  ( ) is expressed in the  nucleus ( ), though ALG-2  also binds annexin 7, peflin, and AIP1/Alix  ( ,   ).	bind
42712	4	11097	6	10	NULL	NULL	NULL	ALG-2	GP		is					apoptosis-linked gene 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_22_20210_s_177	12601007	A more  recently identified ligand of annexin 11, namely the penta-EF-hand protein  ALG-2 (apoptosis-linked gene 2)  ( ) is expressed in the  nucleus ( ), though ALG-2  also binds annexin 7, peflin, and AIP1/Alix  ( ,   ).	bind
42713	5	11097	6	10	NULL	NULL	NULL	ALG-2	GP		is expressed in					nucleus	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_22_20210_s_177	12601007	A more  recently identified ligand of annexin 11, namely the penta-EF-hand protein  ALG-2 (apoptosis-linked gene 2)  ( ) is expressed in the  nucleus ( ), though ALG-2  also binds annexin 7, peflin, and AIP1/Alix  ( ,   ).	bind
42714	6	11097	6	10	NULL	NULL	NULL	ALG-2	GP		is a type of					penta-EF-hand protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_22_20210_s_177	12601007	A more  recently identified ligand of annexin 11, namely the penta-EF-hand protein  ALG-2 (apoptosis-linked gene 2)  ( ) is expressed in the  nucleus ( ), though ALG-2  also binds annexin 7, peflin, and AIP1/Alix  ( ,   ).	bind
42715	7	11097	6	10	NULL	NULL	NULL	ALG-2	GP		is ligand of					annexin 11	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_22_20210_s_177	12601007	A more  recently identified ligand of annexin 11, namely the penta-EF-hand protein  ALG-2 (apoptosis-linked gene 2)  ( ) is expressed in the  nucleus ( ), though ALG-2  also binds annexin 7, peflin, and AIP1/Alix  ( ,   ).	bind
49352	1	11097	7	10	NULL	NULL	NULL	ALG-2	GP		bind					annexin 11	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_22_20210_s_177	12601007	A more  recently identified ligand of annexin 11, namely the penta-EF-hand protein  ALG-2 (apoptosis-linked gene 2)  ( ) is expressed in the  nucleus ( ), though ALG-2  also binds annexin 7, peflin, and AIP1/Alix  ( ,   ).	bind
49353	2	11097	7	10	NULL	NULL	NULL	ALG-2	GP		is expressed in					nucleus	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_22_20210_s_177	12601007	A more  recently identified ligand of annexin 11, namely the penta-EF-hand protein  ALG-2 (apoptosis-linked gene 2)  ( ) is expressed in the  nucleus ( ), though ALG-2  also binds annexin 7, peflin, and AIP1/Alix  ( ,   ).	bind
49354	3	11097	7	10	NULL	NULL	NULL	ALG-2	GP		bind					annexin 7	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_22_20210_s_177	12601007	A more  recently identified ligand of annexin 11, namely the penta-EF-hand protein  ALG-2 (apoptosis-linked gene 2)  ( ) is expressed in the  nucleus ( ), though ALG-2  also binds annexin 7, peflin, and AIP1/Alix  ( ,   ).	bind
49355	4	11097	7	10	NULL	NULL	NULL	ALG-2	GP		bind					peflin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_22_20210_s_177	12601007	A more  recently identified ligand of annexin 11, namely the penta-EF-hand protein  ALG-2 (apoptosis-linked gene 2)  ( ) is expressed in the  nucleus ( ), though ALG-2  also binds annexin 7, peflin, and AIP1/Alix  ( ,   ).	bind
49356	5	11097	7	10	NULL	NULL	NULL	ALG-2	GP		bind					AIP1/Alix 	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_22_20210_s_177	12601007	A more  recently identified ligand of annexin 11, namely the penta-EF-hand protein  ALG-2 (apoptosis-linked gene 2)  ( ) is expressed in the  nucleus ( ), though ALG-2  also binds annexin 7, peflin, and AIP1/Alix  ( ,   ).	bind
49357	6	11097	7	10	NULL	NULL	NULL	ALG-2	GP		is					apoptosis-linked gene 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_22_20210_s_177	12601007	A more  recently identified ligand of annexin 11, namely the penta-EF-hand protein  ALG-2 (apoptosis-linked gene 2)  ( ) is expressed in the  nucleus ( ), though ALG-2  also binds annexin 7, peflin, and AIP1/Alix  ( ,   ).	bind
49358	7	11097	7	10	NULL	NULL	NULL	ALG-2	GP		is a type of					 penta-EF-hand protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_22_20210_s_177	12601007	A more  recently identified ligand of annexin 11, namely the penta-EF-hand protein  ALG-2 (apoptosis-linked gene 2)  ( ) is expressed in the  nucleus ( ), though ALG-2  also binds annexin 7, peflin, and AIP1/Alix  ( ,   ).	bind
42716	1	11098	6	10	NULL	NULL	NULL	CTD peptide	AminoAcid		bind								CTD-binding domain		NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_12_1401_s_41	15964991	A more compact beta-spiral, only 100  Ang  long, and assuming only one beta-turn per repeat, was suggested based on a crystal structure of a CTD peptide bound to a CTD-binding domain ("`compact spiral"`) ( Fig. 1; Meinhart and Cramer 2004 ).	bind
49359	1	11098	7	10	NULL	NULL	NULL	CTD peptide	AminoAcid		bind								CTD-binding domain		NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_12_1401_s_41	15964991	A more compact beta-spiral, only 100  Ang  long, and assuming only one beta-turn per repeat, was suggested based on a crystal structure of a CTD peptide bound to a CTD-binding domain ("`compact spiral"`) ( Fig. 1; Meinhart and Cramer 2004 ).	bind
42717	1	11099	6	10	NULL	NULL	NULL	TnI	GP		interacts with					TnC	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_20_12765_s_137	12239350	A more complex scenario would have the binding of TnT propagating along the polypeptide chain and increasing the interaction between TnI and TnC.	bind
57876	2	11099	6	10	NULL	NULL	NULL	TnT	GP	binding of	propagate along					polypeptide chain	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_20_12765_s_137	12239350	A more complex scenario would have the binding of TnT propagating along the polypeptide chain and increasing the interaction between TnI and TnC.	bind
57877	3	11099	6	10	NULL	NULL	NULL	statement 2	Process		increases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_20_12765_s_137	12239350	A more complex scenario would have the binding of TnT propagating along the polypeptide chain and increasing the interaction between TnI and TnC.	bind
49360	1	11099	7	10	NULL	NULL	NULL	TnI	GP		interact with					TnC	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_20_12765_s_137	12239350	A more complex scenario would have the binding of TnT propagating along the polypeptide chain and increasing the interaction between TnI and TnC.	bind
49361	2	11099	7	10	NULL	NULL	NULL	TnT	GP	binding of	propogate along					polypeptide chain	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_20_12765_s_137	12239350	A more complex scenario would have the binding of TnT propagating along the polypeptide chain and increasing the interaction between TnI and TnC.	bind
49362	3	11099	7	10	NULL	NULL	NULL	statement 2	Process		increase					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_20_12765_s_137	12239350	A more complex scenario would have the binding of TnT propagating along the polypeptide chain and increasing the interaction between TnI and TnC.	bind
42718	1	11100	6	10	NULL	NULL	NULL	Bem1p	GP		is a type of					scaffold protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_20_0_559_s_75	15473852	A more complicated genetic screen identified a third component, Bem1p, a scaffold  protein that binds Cdc24p and Cdc42p ( Bose et al. 2001, Peterson et al. 1994, Zheng et al. 1995).	bind
42719	2	11100	6	10	NULL	NULL	NULL	Bem1p	GP		bind					Cdc24p	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_20_0_559_s_75	15473852	A more complicated genetic screen identified a third component, Bem1p, a scaffold  protein that binds Cdc24p and Cdc42p ( Bose et al. 2001, Peterson et al. 1994, Zheng et al. 1995).	bind
42720	3	11100	6	10	NULL	NULL	NULL	Bem1p	GP		bind					Cdc42p	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_20_0_559_s_75	15473852	A more complicated genetic screen identified a third component, Bem1p, a scaffold  protein that binds Cdc24p and Cdc42p ( Bose et al. 2001, Peterson et al. 1994, Zheng et al. 1995).	bind
49363	1	11100	7	10	NULL	NULL	NULL	Bem1p	GP		bind					Cdc24p	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_20_0_559_s_75	15473852	A more complicated genetic screen identified a third component, Bem1p, a scaffold  protein that binds Cdc24p and Cdc42p ( Bose et al. 2001, Peterson et al. 1994, Zheng et al. 1995).	bind
49364	2	11100	7	10	NULL	NULL	NULL	Bem1p	GP		bind					Cdc42p	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_20_0_559_s_75	15473852	A more complicated genetic screen identified a third component, Bem1p, a scaffold  protein that binds Cdc24p and Cdc42p ( Bose et al. 2001, Peterson et al. 1994, Zheng et al. 1995).	bind
49365	3	11100	7	10	NULL	NULL	NULL	Bem1p	GP		is a type of					scaffold protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_20_0_559_s_75	15473852	A more complicated genetic screen identified a third component, Bem1p, a scaffold  protein that binds Cdc24p and Cdc42p ( Bose et al. 2001, Peterson et al. 1994, Zheng et al. 1995).	bind
42975	1	11101	6	10	NULL	NULL	NULL	estradiol	GP		bind					SHBG	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_34_25920_s_105	10859323	A more detailed analysis (Fig.  3) revealed that the inhibitory effect of zinc on estradiol binding to SHBG could be detected at 10 muM ZnCl2 and increases progressively with increasing ZnCl2 concentrations.	bind
42976	2	11101	6	10	NULL	NULL	NULL	Zinc 	Chemical		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_34_25920_s_105	10859323	A more detailed analysis (Fig.  3) revealed that the inhibitory effect of zinc on estradiol binding to SHBG could be detected at 10 muM ZnCl2 and increases progressively with increasing ZnCl2 concentrations.	bind
49366	1	11101	7	10	NULL	NULL	NULL	estradiol	GP		bind					SHBG	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_34_25920_s_105	10859323	A more detailed analysis (Fig.  3) revealed that the inhibitory effect of zinc on estradiol binding to SHBG could be detected at 10 muM ZnCl2 and increases progressively with increasing ZnCl2 concentrations.	bind
49367	2	11101	7	10	NULL	NULL	NULL	 zinc	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_34_25920_s_105	10859323	A more detailed analysis (Fig.  3) revealed that the inhibitory effect of zinc on estradiol binding to SHBG could be detected at 10 muM ZnCl2 and increases progressively with increasing ZnCl2 concentrations.	bind
42977	1	11102	6	10	NULL	NULL	NULL	Plk1	GP		bind		physically			p53	GP				NULL	cultured cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_6_2093_s_343	16507989	A more detailed analysis of the Plk1/p53 connection showed that Plk1 physically binds to p53 in cultured cells.	bind
49368	1	11102	7	10	NULL	NULL	NULL	Plk1	GP		bind		physically			p53	GP				NULL	cultured cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_6_2093_s_343	16507989	A more detailed analysis of the Plk1/p53 connection showed that Plk1 physically binds to p53 in cultured cells.	bind
43176	1	11103	6	10	NULL	NULL	NULL				bind		specifically	ADF-H domain		F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_1_393_s_227	10637315	A more detailed analysis showed that even the smallest fragment tested in the C-terminal truncation series, the ADF-H domain alone, still bound to F-actin in a specific, saturable manner, although the affinity of binding was reduced compared with the larger fragments (Figure  2B, right panel).	bind
49369	1	11103	7	10	NULL	NULL	NULL				bind		specific	ADF-H domain		F-actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_1_393_s_227	10637315	A more detailed analysis showed that even the smallest fragment tested in the C-terminal truncation series, the ADF-H domain alone, still bound to F-actin in a specific, saturable manner, although the affinity of binding was reduced compared with the larger fragments (Figure  2B, right panel).	bind
42978	1	11104	6	10	NULL	NULL	NULL	F2	NucleicAcid		bind					chimeric TRalpha	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_14_9048_s_180	9083030	A more detailed analysis was carried out by determining the affinities in the binding of F2 to the chimeric TRalphas.	bind
49371	1	11104	7	10	NULL	NULL	NULL	F2 	NucleicAcid		bind					chimeric TRalphas	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_14_9048_s_180	9083030	A more detailed analysis was carried out by determining the affinities in the binding of F2 to the chimeric TRalphas.	bind
43341	1	11105	6	10	NULL	NULL	NULL	LSP1	GP	human	bind			COOH terminal half		F-actin filaments	CellComponent				NULL	intact cells	NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1642_1_17_s_163	12972289	A more detailed study on human LSP1 identified at least three and possibly four  specific regions in the COOH-terminal half of human LSP1 that each individually can  function as an F-actin binding site [ 12], suggesting that binding of LSP1 to the F-actin filaments in intact cells involves  three or four binding sites.	bind
49372	1	11105	7	10	NULL	NULL	NULL	LSP1	GP	human	bind			COOH-terminal half 		F-actin filaments	CellComponent				NULL	intact cells	NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1642_1_17_s_163	12972289	A more detailed study on human LSP1 identified at least three and possibly four  specific regions in the COOH-terminal half of human LSP1 that each individually can  function as an F-actin binding site [ 12], suggesting that binding of LSP1 to the F-actin filaments in intact cells involves  three or four binding sites.	bind
42979	1	11107	6	10	NULL	NULL	NULL	Sir4	GP		stimulates					Sir2	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_16_6931_s_474	15282295	A more detailed understanding of the mechanism of Sir2 activity stimulation by Sir4 and Net1 binding will require a study of the structure of the entire Sir2 protein, both without ligands and in complex with its binding partners.	bind
42980	2	11107	6	10	NULL	NULL	NULL	Net1	GP	binding of	stimulates					Sir2	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_16_6931_s_474	15282295	A more detailed understanding of the mechanism of Sir2 activity stimulation by Sir4 and Net1 binding will require a study of the structure of the entire Sir2 protein, both without ligands and in complex with its binding partners.	bind
49375	1	11107	7	10	NULL	NULL	NULL	Sir4	GP		stimulate					Sir2	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_16_6931_s_474	15282295	A more detailed understanding of the mechanism of Sir2 activity stimulation by Sir4 and Net1 binding will require a study of the structure of the entire Sir2 protein, both without ligands and in complex with its binding partners.	bind
50284	2	11107	7	10	NULL	NULL	NULL	Net1	GP	binding of	stimulates					Sir2	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_16_6931_s_474	15282295	A more detailed understanding of the mechanism of Sir2 activity stimulation by Sir4 and Net1 binding will require a study of the structure of the entire Sir2 protein, both without ligands and in complex with its binding partners.	bind
42981	1	11108	6	10	NULL	NULL	NULL	7S NGF	GP		bind					NGF receptor	GP				NULL	embryonic chicken sensory ganglia	NULL	NULL	NULL	NULL	gw60_annrevneur_24_0_601_s_167	11283322	A more direct approach measured the binding of 7S NGF to the two specific NGF receptors that had just been identified on embryonic chicken sensory ganglia ( Sutter et al 1979).	bind
49376	1	11108	7	10	NULL	NULL	NULL	7S NGF	GP		bind					NGF receptors	GP				NULL	embryonic chicken sensory ganglia	NULL	NULL	NULL	NULL	gw60_annrevneur_24_0_601_s_167	11283322	A more direct approach measured the binding of 7S NGF to the two specific NGF receptors that had just been identified on embryonic chicken sensory ganglia ( Sutter et al 1979).	bind
43344	1	11110	6	10	NULL	NULL	NULL	mu			bind					DG	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_24743_s_25	11328812	A more distantly related group of mu, nu, and PKD-2 isoforms binds DG but is Ca2+-insensitive and may or may not translocate depending on cell type ( 5-7).	bind
43345	2	11110	6	10	NULL	NULL	NULL	nu			bind					DG	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_24743_s_25	11328812	A more distantly related group of mu, nu, and PKD-2 isoforms binds DG but is Ca2+-insensitive and may or may not translocate depending on cell type ( 5-7).	bind
43346	3	11110	6	10	NULL	NULL	NULL	PKD-2 isoforms	GP		bind					DG	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_24743_s_25	11328812	A more distantly related group of mu, nu, and PKD-2 isoforms binds DG but is Ca2+-insensitive and may or may not translocate depending on cell type ( 5-7).	bind
57878	4	11110	6	10	NULL	NULL	NULL	statement 1	Process		is insensitive to					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_24743_s_25	11328812	A more distantly related group of mu, nu, and PKD-2 isoforms binds DG but is Ca2+-insensitive and may or may not translocate depending on cell type ( 5-7).	bind
57879	5	11110	6	10	NULL	NULL	NULL	statement 2	Process		is insensitive to					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_24743_s_25	11328812	A more distantly related group of mu, nu, and PKD-2 isoforms binds DG but is Ca2+-insensitive and may or may not translocate depending on cell type ( 5-7).	bind
57880	6	11110	6	10	NULL	NULL	NULL	statement 3	Process		is insensitive to					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_24743_s_25	11328812	A more distantly related group of mu, nu, and PKD-2 isoforms binds DG but is Ca2+-insensitive and may or may not translocate depending on cell type ( 5-7).	bind
49377	1	11110	7	10	NULL	NULL	NULL	 mu			bind					DG	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_24743_s_25	11328812	A more distantly related group of mu, nu, and PKD-2 isoforms binds DG but is Ca2+-insensitive and may or may not translocate depending on cell type ( 5-7).	bind
49378	2	11110	7	10	NULL	NULL	NULL	nu			bind					DG	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_24743_s_25	11328812	A more distantly related group of mu, nu, and PKD-2 isoforms binds DG but is Ca2+-insensitive and may or may not translocate depending on cell type ( 5-7).	bind
49379	3	11110	7	10	NULL	NULL	NULL	PKD-2 isoforms	GP		bind					DG	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_24743_s_25	11328812	A more distantly related group of mu, nu, and PKD-2 isoforms binds DG but is Ca2+-insensitive and may or may not translocate depending on cell type ( 5-7).	bind
49380	4	11110	7	10	NULL	NULL	NULL	statement 1	Process		is insensitive to					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_24743_s_25	11328812	A more distantly related group of mu, nu, and PKD-2 isoforms binds DG but is Ca2+-insensitive and may or may not translocate depending on cell type ( 5-7).	bind
49381	5	11110	7	10	NULL	NULL	NULL	statement 2	Process		is insensitive to					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_24743_s_25	11328812	A more distantly related group of mu, nu, and PKD-2 isoforms binds DG but is Ca2+-insensitive and may or may not translocate depending on cell type ( 5-7).	bind
49382	6	11110	7	10	NULL	NULL	NULL	statement 3	Process		is insensitive to					Ca2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_27_24743_s_25	11328812	A more distantly related group of mu, nu, and PKD-2 isoforms binds DG but is Ca2+-insensitive and may or may not translocate depending on cell type ( 5-7).	bind
43349	1	11111	6	10	NULL	NULL	NULL	mel-11	GP	worm	is homologous to					MYPT1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_40_37250_s_219	11486008	A more distantly related MYPT1 homologue termed  mel-11 is present in the worm and shares 35% amino acid identity with the higher vertebrate form ( 5,  28,  34,  41).	bind
49386	1	11111	7	10	NULL	NULL	NULL	mel-11	GP	worm	is homologous to					 MYPT1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_40_37250_s_219	11486008	A more distantly related MYPT1 homologue termed  mel-11 is present in the worm and shares 35% amino acid identity with the higher vertebrate form ( 5,  28,  34,  41).	bind
43352	1	11112	6	10	NULL	NULL	NULL	p120ctn	GP		bind					cadherin	GP		juxtamembrane site within the cytoplasmic domain		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_144_3_519_s_21	9971746	A more distantly related protein, p120ctn, also  contains a series of Arm repeats and binds to cadherin (Reynolds et al., 1992  , 1994  ; Shibamoto et al., 1995  ; Staddon et al., 1995  ) at a juxtamembrane site within the cytoplasmic domain of cadherin rather than the more distal  site where beta- and gamma-catenin bind (Ozawa and Kemler,  1998  ; Yap et al., 1998  ). p120ctn does not bind to alpha-catenin  (Daniel and Reynolds, 1995  ) and in nontransformed cells,  only small amounts bind to cadherin (Shibamoto et al.,  1995  ). .	bind
43356	2	11112	6	10	NULL	NULL	NULL	p120ctn	GP		contains								arm repeats		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_144_3_519_s_21	9971746	A more distantly related protein, p120ctn, also  contains a series of Arm repeats and binds to cadherin (Reynolds et al., 1992  , 1994  ; Shibamoto et al., 1995  ; Staddon et al., 1995  ) at a juxtamembrane site within the cytoplasmic domain of cadherin rather than the more distal  site where beta- and gamma-catenin bind (Ozawa and Kemler,  1998  ; Yap et al., 1998  ). p120ctn does not bind to alpha-catenin  (Daniel and Reynolds, 1995  ) and in nontransformed cells,  only small amounts bind to cadherin (Shibamoto et al.,  1995  ). .	bind
43359	3	11112	6	10	NULL	NULL	NULL	beta-catenin	GP		bind					cadherin	GP		distal site		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_144_3_519_s_21	9971746	A more distantly related protein, p120ctn, also  contains a series of Arm repeats and binds to cadherin (Reynolds et al., 1992  , 1994  ; Shibamoto et al., 1995  ; Staddon et al., 1995  ) at a juxtamembrane site within the cytoplasmic domain of cadherin rather than the more distal  site where beta- and gamma-catenin bind (Ozawa and Kemler,  1998  ; Yap et al., 1998  ). p120ctn does not bind to alpha-catenin  (Daniel and Reynolds, 1995  ) and in nontransformed cells,  only small amounts bind to cadherin (Shibamoto et al.,  1995  ). .	bind
43361	4	11112	6	10	NULL	NULL	NULL	gamma-catenin	GP		bind					cadherin	GP		distal site		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_144_3_519_s_21	9971746	A more distantly related protein, p120ctn, also  contains a series of Arm repeats and binds to cadherin (Reynolds et al., 1992  , 1994  ; Shibamoto et al., 1995  ; Staddon et al., 1995  ) at a juxtamembrane site within the cytoplasmic domain of cadherin rather than the more distal  site where beta- and gamma-catenin bind (Ozawa and Kemler,  1998  ; Yap et al., 1998  ). p120ctn does not bind to alpha-catenin  (Daniel and Reynolds, 1995  ) and in nontransformed cells,  only small amounts bind to cadherin (Shibamoto et al.,  1995  ). .	bind
43363	5	11112	6	10	NULL	NULL	NULL	p120ctn	GP		does not bind					alpha-catenin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_144_3_519_s_21	9971746	A more distantly related protein, p120ctn, also  contains a series of Arm repeats and binds to cadherin (Reynolds et al., 1992  , 1994  ; Shibamoto et al., 1995  ; Staddon et al., 1995  ) at a juxtamembrane site within the cytoplasmic domain of cadherin rather than the more distal  site where beta- and gamma-catenin bind (Ozawa and Kemler,  1998  ; Yap et al., 1998  ). p120ctn does not bind to alpha-catenin  (Daniel and Reynolds, 1995  ) and in nontransformed cells,  only small amounts bind to cadherin (Shibamoto et al.,  1995  ). .	bind
43364	6	11112	6	10	NULL	NULL	NULL	p120ctn	GP	small amount	bind					cadherin	GP				NULL	nontransformed cells	NULL	NULL	NULL	NULL	gw60_cellbiol_144_3_519_s_21	9971746	A more distantly related protein, p120ctn, also  contains a series of Arm repeats and binds to cadherin (Reynolds et al., 1992  , 1994  ; Shibamoto et al., 1995  ; Staddon et al., 1995  ) at a juxtamembrane site within the cytoplasmic domain of cadherin rather than the more distal  site where beta- and gamma-catenin bind (Ozawa and Kemler,  1998  ; Yap et al., 1998  ). p120ctn does not bind to alpha-catenin  (Daniel and Reynolds, 1995  ) and in nontransformed cells,  only small amounts bind to cadherin (Shibamoto et al.,  1995  ). .	bind
49388	1	11112	7	10	NULL	NULL	NULL	p120ctn	GP		contains								series of Arm repeats		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_144_3_519_s_21	9971746	A more distantly related protein, p120ctn, also  contains a series of Arm repeats and binds to cadherin (Reynolds et al., 1992  , 1994  ; Shibamoto et al., 1995  ; Staddon et al., 1995  ) at a juxtamembrane site within the cytoplasmic domain of cadherin rather than the more distal  site where beta- and gamma-catenin bind (Ozawa and Kemler,  1998  ; Yap et al., 1998  ). p120ctn does not bind to alpha-catenin  (Daniel and Reynolds, 1995  ) and in nontransformed cells,  only small amounts bind to cadherin (Shibamoto et al.,  1995  ). .	bind
49389	2	11112	7	10	NULL	NULL	NULL	statement 1	Process		bind					cadherin	GP		juxtamembrane site within the cytoplasmic domain		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_144_3_519_s_21	9971746	A more distantly related protein, p120ctn, also  contains a series of Arm repeats and binds to cadherin (Reynolds et al., 1992  , 1994  ; Shibamoto et al., 1995  ; Staddon et al., 1995  ) at a juxtamembrane site within the cytoplasmic domain of cadherin rather than the more distal  site where beta- and gamma-catenin bind (Ozawa and Kemler,  1998  ; Yap et al., 1998  ). p120ctn does not bind to alpha-catenin  (Daniel and Reynolds, 1995  ) and in nontransformed cells,  only small amounts bind to cadherin (Shibamoto et al.,  1995  ). .	bind
49390	3	11112	7	10	NULL	NULL	NULL	beta-catenin	GP		bind					 cadherin	GP		distal site		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_144_3_519_s_21	9971746	A more distantly related protein, p120ctn, also  contains a series of Arm repeats and binds to cadherin (Reynolds et al., 1992  , 1994  ; Shibamoto et al., 1995  ; Staddon et al., 1995  ) at a juxtamembrane site within the cytoplasmic domain of cadherin rather than the more distal  site where beta- and gamma-catenin bind (Ozawa and Kemler,  1998  ; Yap et al., 1998  ). p120ctn does not bind to alpha-catenin  (Daniel and Reynolds, 1995  ) and in nontransformed cells,  only small amounts bind to cadherin (Shibamoto et al.,  1995  ). .	bind
49391	4	11112	7	10	NULL	NULL	NULL	gamma-catenin	GP		bind					cadherin	GP		distal site		NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_144_3_519_s_21	9971746	A more distantly related protein, p120ctn, also  contains a series of Arm repeats and binds to cadherin (Reynolds et al., 1992  , 1994  ; Shibamoto et al., 1995  ; Staddon et al., 1995  ) at a juxtamembrane site within the cytoplasmic domain of cadherin rather than the more distal  site where beta- and gamma-catenin bind (Ozawa and Kemler,  1998  ; Yap et al., 1998  ). p120ctn does not bind to alpha-catenin  (Daniel and Reynolds, 1995  ) and in nontransformed cells,  only small amounts bind to cadherin (Shibamoto et al.,  1995  ). .	bind
49392	5	11112	7	10	NULL	NULL	NULL	 p120ctn	GP		does not bind					alpha-catenin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_144_3_519_s_21	9971746	A more distantly related protein, p120ctn, also  contains a series of Arm repeats and binds to cadherin (Reynolds et al., 1992  , 1994  ; Shibamoto et al., 1995  ; Staddon et al., 1995  ) at a juxtamembrane site within the cytoplasmic domain of cadherin rather than the more distal  site where beta- and gamma-catenin bind (Ozawa and Kemler,  1998  ; Yap et al., 1998  ). p120ctn does not bind to alpha-catenin  (Daniel and Reynolds, 1995  ) and in nontransformed cells,  only small amounts bind to cadherin (Shibamoto et al.,  1995  ). .	bind
49393	6	11112	7	10	NULL	NULL	NULL	 p120ctn	GP		bind					cadherin	GP				NULL	nontransformed cells	NULL	NULL	NULL	NULL	gw60_cellbiol_144_3_519_s_21	9971746	A more distantly related protein, p120ctn, also  contains a series of Arm repeats and binds to cadherin (Reynolds et al., 1992  , 1994  ; Shibamoto et al., 1995  ; Staddon et al., 1995  ) at a juxtamembrane site within the cytoplasmic domain of cadherin rather than the more distal  site where beta- and gamma-catenin bind (Ozawa and Kemler,  1998  ; Yap et al., 1998  ). p120ctn does not bind to alpha-catenin  (Daniel and Reynolds, 1995  ) and in nontransformed cells,  only small amounts bind to cadherin (Shibamoto et al.,  1995  ). .	bind
43633	1	11113	6	10	NULL	NULL	NULL	Pyk2	GP	double mutant	disrupts		completely			ASAP1	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_32_29560_s_157	12771146	A more dramatic effect was observed upon disruption of the first  proline-rich domain of Pyk2 (Pyk2-P717A), and binding of ASAP1 was completely  abolished in the corresponding double mutant.	bind
57881	1	11113	7	10	NULL	NULL	NULL	Pyk2	GP	double mutant	disrupts		completely			ASAP1	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_32_29560_s_157	12771146	A more dramatic effect was observed upon disruption of the first  proline-rich domain of Pyk2 (Pyk2-P717A), and binding of ASAP1 was completely  abolished in the corresponding double mutant.	bind
43158	1	11114	6	10	NULL	NULL	NULL	Nrd1	GP		bind					RNA	NucleicAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_pnas_95_12_6699_s_201	9618475	A more empirical approach e.g., utilizing the selective  in vitro RNA-binding activity of Nrd1 may be necessary to identify the natural targets of Nrd1.	bind
49394	1	11114	7	10	NULL	NULL	NULL	Nrd1	GP		bind					RNA	NucleicAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_pnas_95_12_6699_s_201	9618475	A more empirical approach e.g., utilizing the selective  in vitro RNA-binding activity of Nrd1 may be necessary to identify the natural targets of Nrd1.	bind
43159	1	11115	6	10	NULL	NULL	NULL	DDT	Chemical		bind					EcTS	GP				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_10_981_s_148	11590022	A more extensive search of DDT conformational space than the 500 structures initially used may have more closely predicted the conformation of DDT bound to EcTS.	bind
49395	1	11115	7	10	NULL	NULL	NULL	DDT	Chemical		bind					EcTS	GP				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_8_10_981_s_148	11590022	A more extensive search of DDT conformational space than the 500 structures initially used may have more closely predicted the conformation of DDT bound to EcTS.	bind
43160	1	11116	6	10	NULL	NULL	NULL	CREB	GP		bind					TAT	GP			CRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_23_13716_s_184	8662719	A more extensive study ( 23) indicated that PKA phosphorylation significantly increased the binding of CREB to the tyrosine aminotransferase CRE (TATCRE) and other non-canonical sites, but had less of an effect on the canonical SSCRE.	bind
43161	2	11116	6	10	NULL	NULL	NULL	PKA	GP	phosphorylation of	increases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_23_13716_s_184	8662719	A more extensive study ( 23) indicated that PKA phosphorylation significantly increased the binding of CREB to the tyrosine aminotransferase CRE (TATCRE) and other non-canonical sites, but had less of an effect on the canonical SSCRE.	bind
57882	3	11116	6	10	NULL	NULL	NULL	TAT	GP		is					tyrosine aminotransferase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_23_13716_s_184	8662719	A more extensive study ( 23) indicated that PKA phosphorylation significantly increased the binding of CREB to the tyrosine aminotransferase CRE (TATCRE) and other non-canonical sites, but had less of an effect on the canonical SSCRE.	bind
49396	1	11116	7	10	NULL	NULL	NULL	CREB	GP		bind					TAT	GP			CRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_23_13716_s_184	8662719	A more extensive study ( 23) indicated that PKA phosphorylation significantly increased the binding of CREB to the tyrosine aminotransferase CRE (TATCRE) and other non-canonical sites, but had less of an effect on the canonical SSCRE.	bind
49397	2	11116	7	10	NULL	NULL	NULL	PKA	GP	phosphorylation of	increase					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_23_13716_s_184	8662719	A more extensive study ( 23) indicated that PKA phosphorylation significantly increased the binding of CREB to the tyrosine aminotransferase CRE (TATCRE) and other non-canonical sites, but had less of an effect on the canonical SSCRE.	bind
49398	3	11116	7	10	NULL	NULL	NULL	PKA	GP	phosphorylation of	less effect on							canonical		SSCRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_23_13716_s_184	8662719	A more extensive study ( 23) indicated that PKA phosphorylation significantly increased the binding of CREB to the tyrosine aminotransferase CRE (TATCRE) and other non-canonical sites, but had less of an effect on the canonical SSCRE.	bind
57883	4	11116	7	10	NULL	NULL	NULL	TAT	GP		is					tyrosine aminotransferase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_23_13716_s_184	8662719	A more extensive study ( 23) indicated that PKA phosphorylation significantly increased the binding of CREB to the tyrosine aminotransferase CRE (TATCRE) and other non-canonical sites, but had less of an effect on the canonical SSCRE.	bind
43162	1	11117	6	10	NULL	NULL	NULL	Spo0A	GP		bind					spoIIG	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_1_200_s_181	14679239	A more important role for Spo0A binding to the  spoIIG promoter is illuminated by our model's prediction that the specific interactions between Spo0A and sigmaA that have been demonstrated genetically occur when sigmaA region 4 is located near a sequence centered between positions -33 and -32 of the  spoIIG promoter (Fig.  4B).	bind
43163	2	11117	6	10	NULL	NULL	NULL	Spo0A	GP		interacts with					sigmaA	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_1_200_s_181	14679239	A more important role for Spo0A binding to the  spoIIG promoter is illuminated by our model's prediction that the specific interactions between Spo0A and sigmaA that have been demonstrated genetically occur when sigmaA region 4 is located near a sequence centered between positions -33 and -32 of the  spoIIG promoter (Fig.  4B).	bind
49399	1	11117	7	10	NULL	NULL	NULL	Spo0A	GP		bind					spoIIG	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_1_200_s_181	14679239	A more important role for Spo0A binding to the  spoIIG promoter is illuminated by our model's prediction that the specific interactions between Spo0A and sigmaA that have been demonstrated genetically occur when sigmaA region 4 is located near a sequence centered between positions -33 and -32 of the  spoIIG promoter (Fig.  4B).	bind
49400	2	11117	7	10	NULL	NULL	NULL	Spo0A	GP		interacts with					sigmaA	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_1_200_s_181	14679239	A more important role for Spo0A binding to the  spoIIG promoter is illuminated by our model's prediction that the specific interactions between Spo0A and sigmaA that have been demonstrated genetically occur when sigmaA region 4 is located near a sequence centered between positions -33 and -32 of the  spoIIG promoter (Fig.  4B).	bind
43164	1	11118	6	10	NULL	NULL	NULL	synaptojanin	GP		bind					synaptojanin-binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_13_8710_s_178	9079704	A more interesting explanation may be that the binding of synaptojanin to the 40-kDa synaptojanin-binding protein excludes amphiphysin binding.	bind
43166	2	11118	6	10	NULL	NULL	NULL	statement 1	Process		excludes					amphiphysin	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_13_8710_s_178	9079704	A more interesting explanation may be that the binding of synaptojanin to the 40-kDa synaptojanin-binding protein excludes amphiphysin binding.	bind
49402	1	11118	7	10	NULL	NULL	NULL	synaptojanin	GP		bind					synaptojanin-binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_13_8710_s_178	9079704	A more interesting explanation may be that the binding of synaptojanin to the 40-kDa synaptojanin-binding protein excludes amphiphysin binding.	bind
67683	2	11118	7	10	NULL	0	NULL	statement 1	Process		excludes					amphiphysin	GP	binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_13_8710_s_178	9079704	A more interesting explanation may be that the binding of synaptojanin to the 40-kDa synaptojanin-binding protein excludes amphiphysin binding.	bind
43167	1	11119	6	10	NULL	NULL	NULL	mu1	GP		bind					sigma3	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_5_979_s_156	11230122	A more likely difference between free and mu1-bound forms of sigma3 is disruption of the dimer interface.	bind
49403	1	11119	7	10	NULL	NULL	NULL	mu1	GP		bind					sigma3	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_5_979_s_156	11230122	A more likely difference between free and mu1-bound forms of sigma3 is disruption of the dimer interface.	bind
43168	1	11120	6	10	NULL	NULL	NULL	TFIID	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_22_3007_s_129	9367983	A more likely explanation is that other components of the in vitro transcription reactions (e.g., topoisomerase I) may modify the DNA-binding properties of TFIID and TFIIA, leading to enhanced interactions despite the reduced TATA-Inr spacing.	bind
43169	2	11120	6	10	NULL	NULL	NULL	TFIIA	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_22_3007_s_129	9367983	A more likely explanation is that other components of the in vitro transcription reactions (e.g., topoisomerase I) may modify the DNA-binding properties of TFIID and TFIIA, leading to enhanced interactions despite the reduced TATA-Inr spacing.	bind
43170	3	11120	6	10	NULL	NULL	NULL	topoisomerase  I	GP		is a component of 					transcription reaction	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_genesdev_11_22_3007_s_129	9367983	A more likely explanation is that other components of the in vitro transcription reactions (e.g., topoisomerase I) may modify the DNA-binding properties of TFIID and TFIIA, leading to enhanced interactions despite the reduced TATA-Inr spacing.	bind
43171	4	11120	6	10	NULL	NULL	NULL	statement 3	Process		increases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_22_3007_s_129	9367983	A more likely explanation is that other components of the in vitro transcription reactions (e.g., topoisomerase I) may modify the DNA-binding properties of TFIID and TFIIA, leading to enhanced interactions despite the reduced TATA-Inr spacing.	bind
43172	5	11120	6	10	NULL	NULL	NULL	statement 3	Process		increases					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_22_3007_s_129	9367983	A more likely explanation is that other components of the in vitro transcription reactions (e.g., topoisomerase I) may modify the DNA-binding properties of TFIID and TFIIA, leading to enhanced interactions despite the reduced TATA-Inr spacing.	bind
49404	1	11120	7	10	NULL	NULL	NULL	TFIID	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_22_3007_s_129	9367983	A more likely explanation is that other components of the in vitro transcription reactions (e.g., topoisomerase I) may modify the DNA-binding properties of TFIID and TFIIA, leading to enhanced interactions despite the reduced TATA-Inr spacing.	bind
49405	2	11120	7	10	NULL	NULL	NULL	TFIIA	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_22_3007_s_129	9367983	A more likely explanation is that other components of the in vitro transcription reactions (e.g., topoisomerase I) may modify the DNA-binding properties of TFIID and TFIIA, leading to enhanced interactions despite the reduced TATA-Inr spacing.	bind
49406	3	11120	7	10	NULL	NULL	NULL	topoisomerase I	GP		increase					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_22_3007_s_129	9367983	A more likely explanation is that other components of the in vitro transcription reactions (e.g., topoisomerase I) may modify the DNA-binding properties of TFIID and TFIIA, leading to enhanced interactions despite the reduced TATA-Inr spacing.	bind
49407	4	11120	7	10	NULL	NULL	NULL	topoisomerase I	GP		increase					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_11_22_3007_s_129	9367983	A more likely explanation is that other components of the in vitro transcription reactions (e.g., topoisomerase I) may modify the DNA-binding properties of TFIID and TFIIA, leading to enhanced interactions despite the reduced TATA-Inr spacing.	bind
49408	5	11120	7	10	NULL	NULL	NULL	topoisomerase I	GP		is a component of					transcription reactions	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_genesdev_11_22_3007_s_129	9367983	A more likely explanation is that other components of the in vitro transcription reactions (e.g., topoisomerase I) may modify the DNA-binding properties of TFIID and TFIIA, leading to enhanced interactions despite the reduced TATA-Inr spacing.	bind
43173	1	11121	6	10	NULL	NULL	NULL				bind			Pro-Phe-Lys		OppA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_5_1215_s_192	9495761	A more likely explanation is that Pro-Phe-Lys binds preferentially to OppA rather than MppA.	bind
43174	2	11121	6	10	NULL	NULL	NULL				bind			Pro-Phe-Lys		MppA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_5_1215_s_192	9495761	A more likely explanation is that Pro-Phe-Lys binds preferentially to OppA rather than MppA.	bind
50285	3	11121	6	10	NULL	NULL	NULL	statement 1	Process		is preferred over					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_5_1215_s_192	9495761	A more likely explanation is that Pro-Phe-Lys binds preferentially to OppA rather than MppA.	bind
49410	1	11121	7	10	NULL	NULL	NULL				bind			Pro-Phe-Lys		OppA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_5_1215_s_192	9495761	A more likely explanation is that Pro-Phe-Lys binds preferentially to OppA rather than MppA.	bind
49411	2	11121	7	10	NULL	NULL	NULL				bind			Pro-Phe-Lys		MppA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_5_1215_s_192	9495761	A more likely explanation is that Pro-Phe-Lys binds preferentially to OppA rather than MppA.	bind
49412	3	11121	7	10	NULL	NULL	NULL	statement 1	Process		is preferred than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_5_1215_s_192	9495761	A more likely explanation is that Pro-Phe-Lys binds preferentially to OppA rather than MppA.	bind
43638	1	11122	6	10	NULL	NULL	NULL	NHP6A/B	GP		is required for					nucleoprotein complex	GP	assembly of;; repressive			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_24_6804_s_164	11118215	A more likely function for NHP6A/B at the  CHA1 promoter is that these proteins are required either for assembly of a repressive nucleoprotein complex (e.g. nucleosome) or function as auxiliary co-repressors, facilitating the recruitment/binding of a repressive factor(s) working through chromatin (e.g. histone deacetylase activity).	bind
43640	2	11122	6	10	NULL	NULL	NULL	nucleosome	Chromosome		is a type of					nucleoprotein complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_24_6804_s_164	11118215	A more likely function for NHP6A/B at the  CHA1 promoter is that these proteins are required either for assembly of a repressive nucleoprotein complex (e.g. nucleosome) or function as auxiliary co-repressors, facilitating the recruitment/binding of a repressive factor(s) working through chromatin (e.g. histone deacetylase activity).	bind
43643	3	11122	6	10	NULL	NULL	NULL	NHP6A/B	GP		function as					co-repressors	GP	auxiliary			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_24_6804_s_164	11118215	A more likely function for NHP6A/B at the  CHA1 promoter is that these proteins are required either for assembly of a repressive nucleoprotein complex (e.g. nucleosome) or function as auxiliary co-repressors, facilitating the recruitment/binding of a repressive factor(s) working through chromatin (e.g. histone deacetylase activity).	bind
43645	4	11122	6	10	NULL	NULL	NULL	statement 3	Process		facilitates					repressive factor	GP	recruitment;; binding of			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_24_6804_s_164	11118215	A more likely function for NHP6A/B at the  CHA1 promoter is that these proteins are required either for assembly of a repressive nucleoprotein complex (e.g. nucleosome) or function as auxiliary co-repressors, facilitating the recruitment/binding of a repressive factor(s) working through chromatin (e.g. histone deacetylase activity).	bind
49413	1	11122	7	10	NULL	NULL	NULL	NHP6A/B	GP		is required for					nucleoprotein complex	GP	assembly of;;repressive			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_24_6804_s_164	11118215	A more likely function for NHP6A/B at the  CHA1 promoter is that these proteins are required either for assembly of a repressive nucleoprotein complex (e.g. nucleosome) or function as auxiliary co-repressors, facilitating the recruitment/binding of a repressive factor(s) working through chromatin (e.g. histone deacetylase activity).	bind
49414	2	11122	7	10	NULL	NULL	NULL	NHP6A/B	GP		function as					co-repressors	GP	auxiliary 			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_24_6804_s_164	11118215	A more likely function for NHP6A/B at the  CHA1 promoter is that these proteins are required either for assembly of a repressive nucleoprotein complex (e.g. nucleosome) or function as auxiliary co-repressors, facilitating the recruitment/binding of a repressive factor(s) working through chromatin (e.g. histone deacetylase activity).	bind
49415	3	11122	7	10	NULL	NULL	NULL	NHP6A/B	GP		facilitate					repressive factors	GP	recruitment of;;binding of			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_24_6804_s_164	11118215	A more likely function for NHP6A/B at the  CHA1 promoter is that these proteins are required either for assembly of a repressive nucleoprotein complex (e.g. nucleosome) or function as auxiliary co-repressors, facilitating the recruitment/binding of a repressive factor(s) working through chromatin (e.g. histone deacetylase activity).	bind
49417	5	11122	7	10	NULL	NULL	NULL	nucleosome	Chromosome		is a type of					nucleoprotein complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_24_6804_s_164	11118215	A more likely function for NHP6A/B at the  CHA1 promoter is that these proteins are required either for assembly of a repressive nucleoprotein complex (e.g. nucleosome) or function as auxiliary co-repressors, facilitating the recruitment/binding of a repressive factor(s) working through chromatin (e.g. histone deacetylase activity).	bind
49418	4	11122	7	10	NULL	NULL	NULL	statement 2	Process		occur through					chromatin	Chromosome				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_24_6804_s_164	11118215	A more likely function for NHP6A/B at the  CHA1 promoter is that these proteins are required either for assembly of a repressive nucleoprotein complex (e.g. nucleosome) or function as auxiliary co-repressors, facilitating the recruitment/binding of a repressive factor(s) working through chromatin (e.g. histone deacetylase activity).	bind
43177	1	11123	6	10	NULL	NULL	NULL	Cdc42p	GP		bind					Ste20p	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_1_83_s_172	9009270	A more likely interpretation assumes that Cdc42p binding to Ste20p plays a role in polarized transport of components required for cell-cell adhesion in the tips of mating projections.	bind
43178	2	11123	6	10	NULL	NULL	NULL	components			are required for					cell-cell adhesion	Process				NULL	tips of mating projections	NULL	NULL	NULL	NULL	gw60_embo_16_1_83_s_172	9009270	A more likely interpretation assumes that Cdc42p binding to Ste20p plays a role in polarized transport of components required for cell-cell adhesion in the tips of mating projections.	bind
43179	3	11123	6	10	NULL	NULL	NULL	statement 1	Process		plays a role in					statement 2	Process	polarized;; transport of 			NULL		NULL	NULL	NULL	NULL	gw60_embo_16_1_83_s_172	9009270	A more likely interpretation assumes that Cdc42p binding to Ste20p plays a role in polarized transport of components required for cell-cell adhesion in the tips of mating projections.	bind
49419	1	11123	7	10	NULL	NULL	NULL	Cdc42p	GP		bind					Ste20p 	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_1_83_s_172	9009270	A more likely interpretation assumes that Cdc42p binding to Ste20p plays a role in polarized transport of components required for cell-cell adhesion in the tips of mating projections.	bind
49420	2	11123	7	10	NULL	NULL	NULL	statement 1	Process		plays a role in					components		polarized;;transport of			NULL		NULL	NULL	NULL	NULL	gw60_embo_16_1_83_s_172	9009270	A more likely interpretation assumes that Cdc42p binding to Ste20p plays a role in polarized transport of components required for cell-cell adhesion in the tips of mating projections.	bind
49421	3	11123	7	10	NULL	NULL	NULL	statement 2	Process		is required for					cell-cell adhesion	Process				NULL	tips of mating projections	NULL	NULL	NULL	NULL	gw60_embo_16_1_83_s_172	9009270	A more likely interpretation assumes that Cdc42p binding to Ste20p plays a role in polarized transport of components required for cell-cell adhesion in the tips of mating projections.	bind
43647	1	11124	6	10	NULL	NULL	NULL	gamma complex	GP		bind					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5131_s_200	10487764	A more likely possibility is that ATP binding is fast, but the gamma complex is not committed to hydrolyzing every ATP it binds (i.e. ATP dissociation competes effectively with ATP hydrolysis, when beta and DNA are absent).	bind
43649	2	11124	6	10	NULL	NULL	NULL	ATP	Chemical	dissociation of	competes with					ATP	Chemical	hydrolysis of			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5131_s_200	10487764	A more likely possibility is that ATP binding is fast, but the gamma complex is not committed to hydrolyzing every ATP it binds (i.e. ATP dissociation competes effectively with ATP hydrolysis, when beta and DNA are absent).	bind
43651	3	11124	6	10	NULL	NULL	NULL	statement 2	Process		occurs in absence of					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5131_s_200	10487764	A more likely possibility is that ATP binding is fast, but the gamma complex is not committed to hydrolyzing every ATP it binds (i.e. ATP dissociation competes effectively with ATP hydrolysis, when beta and DNA are absent).	bind
43652	4	11124	6	10	NULL	NULL	NULL	statement 2	Process		occurs in absence of					beta					NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5131_s_200	10487764	A more likely possibility is that ATP binding is fast, but the gamma complex is not committed to hydrolyzing every ATP it binds (i.e. ATP dissociation competes effectively with ATP hydrolysis, when beta and DNA are absent).	bind
49422	1	11124	7	10	NULL	NULL	NULL	ATP	Chemical	dissociation of	compete with		effectively			ATP	Chemical	hydrolysis of			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5131_s_200	10487764	A more likely possibility is that ATP binding is fast, but the gamma complex is not committed to hydrolyzing every ATP it binds (i.e. ATP dissociation competes effectively with ATP hydrolysis, when beta and DNA are absent).	bind
49423	2	11124	7	10	NULL	NULL	NULL	statement 1	Process		in absence of					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5131_s_200	10487764	A more likely possibility is that ATP binding is fast, but the gamma complex is not committed to hydrolyzing every ATP it binds (i.e. ATP dissociation competes effectively with ATP hydrolysis, when beta and DNA are absent).	bind
49424	3	11124	7	10	NULL	NULL	NULL	statement 1	Process		in absence of					beta					NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5131_s_200	10487764	A more likely possibility is that ATP binding is fast, but the gamma complex is not committed to hydrolyzing every ATP it binds (i.e. ATP dissociation competes effectively with ATP hydrolysis, when beta and DNA are absent).	bind
50304	4	11124	7	10	NULL	NULL	NULL	gamma complex	GP		bind					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_18_5131_s_200	10487764	A more likely possibility is that ATP binding is fast, but the gamma complex is not committed to hydrolyzing every ATP it binds (i.e. ATP dissociation competes effectively with ATP hydrolysis, when beta and DNA are absent).	bind
43181	1	11125	6	10	NULL	NULL	NULL	RRD proteins	GP	loss of	affects					PPH21	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_17_2138_s_250	12952889	A more likely possibility is that loss of the RRD proteins affects other  proteins in addition to PPH21 and PPH22.	bind
43182	2	11125	6	10	NULL	NULL	NULL	RRD proteins	GP	loss of	affects					PPH22	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_17_2138_s_250	12952889	A more likely possibility is that loss of the RRD proteins affects other  proteins in addition to PPH21 and PPH22.	bind
49426	1	11125	7	10	NULL	NULL	NULL	RRD proteins	GP	loss of	affects					 PPH21	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_17_2138_s_250	12952889	A more likely possibility is that loss of the RRD proteins affects other  proteins in addition to PPH21 and PPH22.	bind
49427	2	11125	7	10	NULL	NULL	NULL	RRD proteins	GP	loss of	affects					PPH22	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_17_2138_s_250	12952889	A more likely possibility is that loss of the RRD proteins affects other  proteins in addition to PPH21 and PPH22.	bind
43183	1	11126	6	10	NULL	NULL	NULL	E2	GP		contains								lipoyl domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_23_14130_s_238	9603912	A more likely prospect is that E1b, which is bound to an E2 containing two lipoyl domains, makes E1b a better substrate than free E1b for an unbound PDP, particularly when located next to a nonlipoylated L2.	bind
43184	2	11126	6	10	NULL	NULL	NULL	E1b	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_23_14130_s_238	9603912	A more likely prospect is that E1b, which is bound to an E2 containing two lipoyl domains, makes E1b a better substrate than free E1b for an unbound PDP, particularly when located next to a nonlipoylated L2.	bind
43655	3	11126	6	10	NULL	NULL	NULL	statement 2	Process		acts as a substrate for					PDP	GP	unbound			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_23_14130_s_238	9603912	A more likely prospect is that E1b, which is bound to an E2 containing two lipoyl domains, makes E1b a better substrate than free E1b for an unbound PDP, particularly when located next to a nonlipoylated L2.	bind
57884	4	11126	6	10	NULL	NULL	NULL	E1b	GP	free	is a substrate for					PDP	GP	unbound			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_23_14130_s_238	9603912	A more likely prospect is that E1b, which is bound to an E2 containing two lipoyl domains, makes E1b a better substrate than free E1b for an unbound PDP, particularly when located next to a nonlipoylated L2.	bind
57885	5	11126	6	10	NULL	NULL	NULL	statement 3	Process		better than					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_23_14130_s_238	9603912	A more likely prospect is that E1b, which is bound to an E2 containing two lipoyl domains, makes E1b a better substrate than free E1b for an unbound PDP, particularly when located next to a nonlipoylated L2.	bind
49428	1	11126	7	10	NULL	NULL	NULL	E2	GP		contains								lipoyl domains		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_23_14130_s_238	9603912	A more likely prospect is that E1b, which is bound to an E2 containing two lipoyl domains, makes E1b a better substrate than free E1b for an unbound PDP, particularly when located next to a nonlipoylated L2.	bind
49429	2	11126	7	10	NULL	NULL	NULL	E1b	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_23_14130_s_238	9603912	A more likely prospect is that E1b, which is bound to an E2 containing two lipoyl domains, makes E1b a better substrate than free E1b for an unbound PDP, particularly when located next to a nonlipoylated L2.	bind
49430	3	11126	7	10	NULL	NULL	NULL	statement 2	Process		substrate for					PDP	GP	unbound 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_23_14130_s_238	9603912	A more likely prospect is that E1b, which is bound to an E2 containing two lipoyl domains, makes E1b a better substrate than free E1b for an unbound PDP, particularly when located next to a nonlipoylated L2.	bind
49431	4	11126	7	10	NULL	NULL	NULL	E1b	GP	free	substrate for					PDP	GP	unbound			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_23_14130_s_238	9603912	A more likely prospect is that E1b, which is bound to an E2 containing two lipoyl domains, makes E1b a better substrate than free E1b for an unbound PDP, particularly when located next to a nonlipoylated L2.	bind
49432	5	11126	7	10	NULL	NULL	NULL	statement 3	Process		is better than					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_23_14130_s_238	9603912	A more likely prospect is that E1b, which is bound to an E2 containing two lipoyl domains, makes E1b a better substrate than free E1b for an unbound PDP, particularly when located next to a nonlipoylated L2.	bind
43185	1	11127	6	10	NULL	NULL	NULL	PtdIns-3,4,5-P3	Chemical		bind								PH domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_111_3_293_s_81	12419241	A more likely scenario is that after initial membrane translocation and activation via PtdIns-3,4,5-P3 binding to its PH domain, PKB dissociates from the plasma membrane, thus freeing its PH domain to interact with protein ligands such as TCL1.	bind
43666	2	11127	6	10	NULL	NULL	NULL	TCL1	GP		interacts with								PH domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_111_3_293_s_81	12419241	A more likely scenario is that after initial membrane translocation and activation via PtdIns-3,4,5-P3 binding to its PH domain, PKB dissociates from the plasma membrane, thus freeing its PH domain to interact with protein ligands such as TCL1.	bind
43668	3	11127	6	10	NULL	NULL	NULL	statement 1	Process		leads to					membrane	CellComponent	translocation of			NULL		NULL	NULL	NULL	NULL	gw60_cell_111_3_293_s_81	12419241	A more likely scenario is that after initial membrane translocation and activation via PtdIns-3,4,5-P3 binding to its PH domain, PKB dissociates from the plasma membrane, thus freeing its PH domain to interact with protein ligands such as TCL1.	bind
43671	4	11127	6	10	NULL	NULL	NULL	statement 1	Process		leads to					membrane	CellComponent	activation of			NULL		NULL	NULL	NULL	NULL	gw60_cell_111_3_293_s_81	12419241	A more likely scenario is that after initial membrane translocation and activation via PtdIns-3,4,5-P3 binding to its PH domain, PKB dissociates from the plasma membrane, thus freeing its PH domain to interact with protein ligands such as TCL1.	bind
43676	5	11127	6	10	NULL	NULL	NULL	PKB	GP		dissociates from					plasma membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cell_111_3_293_s_81	12419241	A more likely scenario is that after initial membrane translocation and activation via PtdIns-3,4,5-P3 binding to its PH domain, PKB dissociates from the plasma membrane, thus freeing its PH domain to interact with protein ligands such as TCL1.	bind
49434	1	11127	7	10	NULL	NULL	NULL	PKB	GP		translocates to					membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cell_111_3_293_s_81	12419241	A more likely scenario is that after initial membrane translocation and activation via PtdIns-3,4,5-P3 binding to its PH domain, PKB dissociates from the plasma membrane, thus freeing its PH domain to interact with protein ligands such as TCL1.	bind
49435	2	11127	7	10	NULL	NULL	NULL	PKB	GP		bind			PH domain		PtdIns-3,4,5-P3	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_111_3_293_s_81	12419241	A more likely scenario is that after initial membrane translocation and activation via PtdIns-3,4,5-P3 binding to its PH domain, PKB dissociates from the plasma membrane, thus freeing its PH domain to interact with protein ligands such as TCL1.	bind
49436	3	11127	7	10	NULL	NULL	NULL	statement 2	Process		leads to					PKB	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_cell_111_3_293_s_81	12419241	A more likely scenario is that after initial membrane translocation and activation via PtdIns-3,4,5-P3 binding to its PH domain, PKB dissociates from the plasma membrane, thus freeing its PH domain to interact with protein ligands such as TCL1.	bind
49437	4	11127	7	10	NULL	NULL	NULL	PKB	GP		dissociates from					plasma membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cell_111_3_293_s_81	12419241	A more likely scenario is that after initial membrane translocation and activation via PtdIns-3,4,5-P3 binding to its PH domain, PKB dissociates from the plasma membrane, thus freeing its PH domain to interact with protein ligands such as TCL1.	bind
49438	5	11127	7	10	NULL	NULL	NULL	statement 4	Process		release					PKB	GP		PH domain		NULL		NULL	NULL	NULL	NULL	gw60_cell_111_3_293_s_81	12419241	A more likely scenario is that after initial membrane translocation and activation via PtdIns-3,4,5-P3 binding to its PH domain, PKB dissociates from the plasma membrane, thus freeing its PH domain to interact with protein ligands such as TCL1.	bind
49439	6	11127	7	10	NULL	NULL	NULL	PKB	GP		interacts with			PH domain		TCL1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_111_3_293_s_81	12419241	A more likely scenario is that after initial membrane translocation and activation via PtdIns-3,4,5-P3 binding to its PH domain, PKB dissociates from the plasma membrane, thus freeing its PH domain to interact with protein ligands such as TCL1.	bind
49440	7	11127	7	10	NULL	NULL	NULL	statement 4	Process		occurs after					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_111_3_293_s_81	12419241	A more likely scenario is that after initial membrane translocation and activation via PtdIns-3,4,5-P3 binding to its PH domain, PKB dissociates from the plasma membrane, thus freeing its PH domain to interact with protein ligands such as TCL1.	bind
49441	8	11127	7	10	NULL	NULL	NULL	statement 4	Process		occurs after					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_111_3_293_s_81	12419241	A more likely scenario is that after initial membrane translocation and activation via PtdIns-3,4,5-P3 binding to its PH domain, PKB dissociates from the plasma membrane, thus freeing its PH domain to interact with protein ligands such as TCL1.	bind
43186	1	11128	6	10	NULL	NULL	NULL	HDL	Chemical		bind					SR-BI	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_29993_s_244	11001950	A more parsimonious model is that KKB-1 blocks SR-BI-mediated [3]cholesterol efflux to HDL by blocking HDL binding to SR-BI.	bind
43187	2	11128	6	10	NULL	NULL	NULL	cholesterol	Chemical		effluxes					HDL	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_29993_s_244	11001950	A more parsimonious model is that KKB-1 blocks SR-BI-mediated [3]cholesterol efflux to HDL by blocking HDL binding to SR-BI.	bind
43188	3	11128	6	10	NULL	NULL	NULL	SR-BI	GP		mediates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_29993_s_244	11001950	A more parsimonious model is that KKB-1 blocks SR-BI-mediated [3]cholesterol efflux to HDL by blocking HDL binding to SR-BI.	bind
43189	4	11128	6	10	NULL	NULL	NULL	KKB-1	GP		blocks					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_29993_s_244	11001950	A more parsimonious model is that KKB-1 blocks SR-BI-mediated [3]cholesterol efflux to HDL by blocking HDL binding to SR-BI.	bind
43190	5	11128	6	10	NULL	NULL	NULL	statement 4	Process		occurs by blocking					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_29993_s_244	11001950	A more parsimonious model is that KKB-1 blocks SR-BI-mediated [3]cholesterol efflux to HDL by blocking HDL binding to SR-BI.	bind
49442	1	11128	7	10	NULL	NULL	NULL	HDL	Chemical		bind					SR-BI	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_29993_s_244	11001950	A more parsimonious model is that KKB-1 blocks SR-BI-mediated [3]cholesterol efflux to HDL by blocking HDL binding to SR-BI.	bind
49443	2	11128	7	10	NULL	NULL	NULL	cholesterol	Chemical		efflux to					HDL	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_29993_s_244	11001950	A more parsimonious model is that KKB-1 blocks SR-BI-mediated [3]cholesterol efflux to HDL by blocking HDL binding to SR-BI.	bind
49444	3	11128	7	10	NULL	NULL	NULL	SR-BI	GP		mediates					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_29993_s_244	11001950	A more parsimonious model is that KKB-1 blocks SR-BI-mediated [3]cholesterol efflux to HDL by blocking HDL binding to SR-BI.	bind
49445	4	11128	7	10	NULL	NULL	NULL	KKB-1 	GP		blocks					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_29993_s_244	11001950	A more parsimonious model is that KKB-1 blocks SR-BI-mediated [3]cholesterol efflux to HDL by blocking HDL binding to SR-BI.	bind
49446	5	11128	7	10	NULL	NULL	NULL	KKB-1 	GP		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_29993_s_244	11001950	A more parsimonious model is that KKB-1 blocks SR-BI-mediated [3]cholesterol efflux to HDL by blocking HDL binding to SR-BI.	bind
49447	6	11128	7	10	NULL	NULL	NULL	statement 4	Process		occur by					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_29993_s_244	11001950	A more parsimonious model is that KKB-1 blocks SR-BI-mediated [3]cholesterol efflux to HDL by blocking HDL binding to SR-BI.	bind
43191	1	11133	6	10	NULL	NULL	NULL	GABA	Chemical		bind					hydra membranes	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_85_3_979_s_85	9639289	A more pronounced increase in [3]GABA binding to  Hydra membranes was apparent in the presence of general anaesthetics ( Fig. 1A).	bind
49453	1	11133	7	10	NULL	NULL	NULL	GABA	Chemical		bind					hydra membranes	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_85_3_979_s_85	9639289	A more pronounced increase in [3]GABA binding to  Hydra membranes was apparent in the presence of general anaesthetics ( Fig. 1A).	bind
43192	1	11134	6	10	NULL	NULL	NULL	guanine nucleotides	NucleicAcid		bind					Ras protein	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_45_46715_s_31	15339905	A more recent assay to analyze quantitatively the guanine nucleotides bound to the Ras proteins  in vivo was described by Taylor and Shalloway ( ) and exploits the known specificity of the interaction between Ras-GTP and the Ras-binding domain (RBD) of Raf-1 to detect activated Ras.	bind
43193	2	11134	6	10	NULL	NULL	NULL	Ras-GTP	GP		interacts with					Raf-1	GP		RBD		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_45_46715_s_31	15339905	A more recent assay to analyze quantitatively the guanine nucleotides bound to the Ras proteins  in vivo was described by Taylor and Shalloway ( ) and exploits the known specificity of the interaction between Ras-GTP and the Ras-binding domain (RBD) of Raf-1 to detect activated Ras.	bind
43194	3	11134	6	10	NULL	NULL	NULL	RBD	AminoAcid		is					Ras-binding domain	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_45_46715_s_31	15339905	A more recent assay to analyze quantitatively the guanine nucleotides bound to the Ras proteins  in vivo was described by Taylor and Shalloway ( ) and exploits the known specificity of the interaction between Ras-GTP and the Ras-binding domain (RBD) of Raf-1 to detect activated Ras.	bind
49455	1	11134	7	10	NULL	NULL	NULL	guanine nucleotides	NucleicAcid		bind					Ras proteins	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_45_46715_s_31	15339905	A more recent assay to analyze quantitatively the guanine nucleotides bound to the Ras proteins  in vivo was described by Taylor and Shalloway ( ) and exploits the known specificity of the interaction between Ras-GTP and the Ras-binding domain (RBD) of Raf-1 to detect activated Ras.	bind
49456	2	11134	7	10	NULL	NULL	NULL	Ras-GTP 	GP		interacts with					Raf-1	GP		RBD		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_45_46715_s_31	15339905	A more recent assay to analyze quantitatively the guanine nucleotides bound to the Ras proteins  in vivo was described by Taylor and Shalloway ( ) and exploits the known specificity of the interaction between Ras-GTP and the Ras-binding domain (RBD) of Raf-1 to detect activated Ras.	bind
49457	3	11134	7	10	NULL	NULL	NULL	RBD	AminoAcid		is					Ras-binding domain	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_45_46715_s_31	15339905	A more recent assay to analyze quantitatively the guanine nucleotides bound to the Ras proteins  in vivo was described by Taylor and Shalloway ( ) and exploits the known specificity of the interaction between Ras-GTP and the Ras-binding domain (RBD) of Raf-1 to detect activated Ras.	bind
49458	4	11134	7	10	NULL	NULL	NULL	statement 2	Process		detects					Ras	GP	activated			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_45_46715_s_31	15339905	A more recent assay to analyze quantitatively the guanine nucleotides bound to the Ras proteins  in vivo was described by Taylor and Shalloway ( ) and exploits the known specificity of the interaction between Ras-GTP and the Ras-binding domain (RBD) of Raf-1 to detect activated Ras.	bind
43220	1	11135	6	10	NULL	NULL	NULL	ARS1	GP		is assembled into					chromatin	Chromosome				NULL	in vitro chromatin assembly extract	NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_142_s_321	15020055	A more recent biochemical study of ORC and Abf1p binding to  ARS1 assembled into chromatin in an in vitro chromatin assembly extract confirms and extends  these findings [ 113].	bind
43221	2	11135	6	10	NULL	NULL	NULL	ORC	NucleicAcid		bind					statement 1	Process				NULL	in vitro chromatin assembly extract	NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_142_s_321	15020055	A more recent biochemical study of ORC and Abf1p binding to  ARS1 assembled into chromatin in an in vitro chromatin assembly extract confirms and extends  these findings [ 113].	bind
43222	3	11135	6	10	NULL	NULL	NULL	Abf1p	GP		bind					statement 1	Process				NULL	in vitro chromatin assembly extract	NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_142_s_321	15020055	A more recent biochemical study of ORC and Abf1p binding to  ARS1 assembled into chromatin in an in vitro chromatin assembly extract confirms and extends  these findings [ 113].	bind
49459	1	11135	7	10	NULL	NULL	NULL	ORC 	NucleicAcid		bind					ARS1	GP				NULL	in vitro chromatin assembly extract	NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_142_s_321	15020055	A more recent biochemical study of ORC and Abf1p binding to  ARS1 assembled into chromatin in an in vitro chromatin assembly extract confirms and extends  these findings [ 113].	bind
49460	2	11135	7	10	NULL	NULL	NULL	Abf1p	GP		bind					ARS1	GP				NULL	in vitro chromatin assembly extract	NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_142_s_321	15020055	A more recent biochemical study of ORC and Abf1p binding to  ARS1 assembled into chromatin in an in vitro chromatin assembly extract confirms and extends  these findings [ 113].	bind
49461	3	11135	7	10	NULL	NULL	NULL	ARS1	GP		assembled into					chromatin	Chromosome				NULL	in vitro chromatin assembly extract	NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_142_s_321	15020055	A more recent biochemical study of ORC and Abf1p binding to  ARS1 assembled into chromatin in an in vitro chromatin assembly extract confirms and extends  these findings [ 113].	bind
43975	1	11136	6	10	NULL	NULL	NULL	L-CPTI	GP		are critical for			first 18 N-terminal amino acid residues		malonyl-CoA	GP	inhibiton of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_14_9421_s_157	10092622	A more recent detailed deletion mutation analysis study of the 129 N-terminal amino acid residues of the yeast-expressed L-CPTI from our laboratory clearly demonstrated that residues critical for malonyl-CoA inhibition and binding of L-CPTI are located within the conserved first 18 N-terminal amino acid residues of the enzyme ( 14).	bind
43976	2	11136	6	10	NULL	NULL	NULL	L-CPTI	GP		are critical for			first 18 N-terminal amino acid residues		L-CPTI	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_14_9421_s_157	10092622	A more recent detailed deletion mutation analysis study of the 129 N-terminal amino acid residues of the yeast-expressed L-CPTI from our laboratory clearly demonstrated that residues critical for malonyl-CoA inhibition and binding of L-CPTI are located within the conserved first 18 N-terminal amino acid residues of the enzyme ( 14).	bind
50305	1	11136	7	10	NULL	NULL	NULL	L-CPTI	GP		are critical for			first 18 N-terminal amino acid residues		malonyl-CoA	GP	inhibiton of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_14_9421_s_157	10092622	A more recent detailed deletion mutation analysis study of the 129 N-terminal amino acid residues of the yeast-expressed L-CPTI from our laboratory clearly demonstrated that residues critical for malonyl-CoA inhibition and binding of L-CPTI are located within the conserved first 18 N-terminal amino acid residues of the enzyme ( 14).	bind
50306	2	11136	7	10	NULL	NULL	NULL	L-CPTI	GP		are critical for			first 18 N-terminal amino acid residues		L-CPTI	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_14_9421_s_157	10092622	A more recent detailed deletion mutation analysis study of the 129 N-terminal amino acid residues of the yeast-expressed L-CPTI from our laboratory clearly demonstrated that residues critical for malonyl-CoA inhibition and binding of L-CPTI are located within the conserved first 18 N-terminal amino acid residues of the enzyme ( 14).	bind
43223	1	11137	6	10	NULL	NULL	NULL	Sir2Tm	GP	wild type	bind					NAD+	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_75_0_435_s_472	16756498	A more recent structure of a ternary complex containing wild-type  Sir2Tm bound to NAD+ and acetylated peptide (K. Hoff, J. Avalos, K. Sens, and C. Wolberger, manuscript  submitted) provides further insights into the true nature of the Michaelis complex.	bind
43224	2	11137	6	10	NULL	NULL	NULL	Sir2Tm	GP	wild type	bind					peptide	AminoAcid	acetylated			NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_75_0_435_s_472	16756498	A more recent structure of a ternary complex containing wild-type  Sir2Tm bound to NAD+ and acetylated peptide (K. Hoff, J. Avalos, K. Sens, and C. Wolberger, manuscript  submitted) provides further insights into the true nature of the Michaelis complex.	bind
49465	1	11137	7	10	NULL	NULL	NULL	Sir2Tm	GP	wild-type	bind					NAD+	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_75_0_435_s_472	16756498	A more recent structure of a ternary complex containing wild-type  Sir2Tm bound to NAD+ and acetylated peptide (K. Hoff, J. Avalos, K. Sens, and C. Wolberger, manuscript  submitted) provides further insights into the true nature of the Michaelis complex.	bind
49466	2	11137	7	10	NULL	NULL	NULL	Sir2Tm	GP	wild-type	bind					peptide	AminoAcid	acetylated			NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_75_0_435_s_472	16756498	A more recent structure of a ternary complex containing wild-type  Sir2Tm bound to NAD+ and acetylated peptide (K. Hoff, J. Avalos, K. Sens, and C. Wolberger, manuscript  submitted) provides further insights into the true nature of the Michaelis complex.	bind
43225	1	11138	6	10	NULL	NULL	NULL	Oct-1	GP		does not bind					HIV-1	Organism			LTR	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_13_4285_s_586	16061936	A more recent study contrasts with the latter one and demonstrates that Oct-1 and Oct-2 fail to bind the HIV-1 LTR, and that overexpression of Oct proteins has no effect on HIV-1 transcription or replication in primary human CD4+ T-cells ( ).	bind
43226	2	11138	6	10	NULL	NULL	NULL	Oct-2	GP		does not bind					HIV-1	Organism			LTR	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_13_4285_s_586	16061936	A more recent study contrasts with the latter one and demonstrates that Oct-1 and Oct-2 fail to bind the HIV-1 LTR, and that overexpression of Oct proteins has no effect on HIV-1 transcription or replication in primary human CD4+ T-cells ( ).	bind
43227	3	11138	6	10	NULL	NULL	NULL	Oct proteins	GP	overexpression of	has no effect on					HIV-1	Organism	transcription of			NULL	primary human CD4+ T-cells	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_13_4285_s_586	16061936	A more recent study contrasts with the latter one and demonstrates that Oct-1 and Oct-2 fail to bind the HIV-1 LTR, and that overexpression of Oct proteins has no effect on HIV-1 transcription or replication in primary human CD4+ T-cells ( ).	bind
43228	4	11138	6	10	NULL	NULL	NULL	Oct proteins	GP	overexpression of	has no effect on					HIV-1	Organism	replication of 			NULL	primary human CD4+ T-cells	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_13_4285_s_586	16061936	A more recent study contrasts with the latter one and demonstrates that Oct-1 and Oct-2 fail to bind the HIV-1 LTR, and that overexpression of Oct proteins has no effect on HIV-1 transcription or replication in primary human CD4+ T-cells ( ).	bind
49467	1	11138	7	10	NULL	NULL	NULL	Oct-1 	GP		does not bind					HIV-1	Organism			LTR	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_13_4285_s_586	16061936	A more recent study contrasts with the latter one and demonstrates that Oct-1 and Oct-2 fail to bind the HIV-1 LTR, and that overexpression of Oct proteins has no effect on HIV-1 transcription or replication in primary human CD4+ T-cells ( ).	bind
49468	2	11138	7	10	NULL	NULL	NULL	Oct-2	GP		does not bind					HIV-1	Organism			LTR	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_13_4285_s_586	16061936	A more recent study contrasts with the latter one and demonstrates that Oct-1 and Oct-2 fail to bind the HIV-1 LTR, and that overexpression of Oct proteins has no effect on HIV-1 transcription or replication in primary human CD4+ T-cells ( ).	bind
49469	3	11138	7	10	NULL	NULL	NULL	Oct proteins	GP	overexpression of 	does not affect					HIV-1	Organism	transcription of			NULL	primary human CD4+ T-cells	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_13_4285_s_586	16061936	A more recent study contrasts with the latter one and demonstrates that Oct-1 and Oct-2 fail to bind the HIV-1 LTR, and that overexpression of Oct proteins has no effect on HIV-1 transcription or replication in primary human CD4+ T-cells ( ).	bind
49470	4	11138	7	10	NULL	NULL	NULL	Oct proteins 	GP	overexpression of	does not affect					HIV-1	Organism	replication of			NULL	primary human CD4+ T-cells	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_13_4285_s_586	16061936	A more recent study contrasts with the latter one and demonstrates that Oct-1 and Oct-2 fail to bind the HIV-1 LTR, and that overexpression of Oct proteins has no effect on HIV-1 transcription or replication in primary human CD4+ T-cells ( ).	bind
43229	1	11139	6	10	NULL	NULL	NULL	BvgA	GP	phosphorylated	bind					bvgR	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_187_5_1648_s_26	15716435	A more recent study demonstrated that expression of BvgR is activated by the binding of phosphorylated BvgA to the  bvgR promoter ( ).	bind
43230	2	11139	6	10	NULL	NULL	NULL	BvgR	GP	expression of	is activated by					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_187_5_1648_s_26	15716435	A more recent study demonstrated that expression of BvgR is activated by the binding of phosphorylated BvgA to the  bvgR promoter ( ).	bind
49471	1	11139	7	10	NULL	NULL	NULL	BvgA	GP	phosphorylated 	bind					bvgR	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_187_5_1648_s_26	15716435	A more recent study demonstrated that expression of BvgR is activated by the binding of phosphorylated BvgA to the  bvgR promoter ( ).	bind
49472	2	11139	7	10	NULL	NULL	NULL	statement 1	Process		leads to					 BvgR 	GP	activation of;;expression of			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_187_5_1648_s_26	15716435	A more recent study demonstrated that expression of BvgR is activated by the binding of phosphorylated BvgA to the  bvgR promoter ( ).	bind
43231	1	11140	6	10	NULL	NULL	NULL	aggrecan	GP		bind					hyaluronan	GP				NULL	bovine cartilage explants	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_9_6321_s_23	10692431	A more recent study demonstrated that the extent of tissue compression, with the concomitant changes in proteoglycan concentration and pH of the extracellular matrix, could influence the hyaluronan binding properties of aggrecan in bovine cartilage explants ( 14).	bind
43232	2	11140	6	10	NULL	NULL	NULL	proteoglycan	GP	change in concentration of	influence					statement 1	Process				NULL	bovine cartilage explants	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_9_6321_s_23	10692431	A more recent study demonstrated that the extent of tissue compression, with the concomitant changes in proteoglycan concentration and pH of the extracellular matrix, could influence the hyaluronan binding properties of aggrecan in bovine cartilage explants ( 14).	bind
43233	3	11140	6	10	NULL	NULL	NULL	extracellular matrix	CellComponent	change in pH of	influence		could			statement 1	Process				NULL	bovine cartilage explants	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_9_6321_s_23	10692431	A more recent study demonstrated that the extent of tissue compression, with the concomitant changes in proteoglycan concentration and pH of the extracellular matrix, could influence the hyaluronan binding properties of aggrecan in bovine cartilage explants ( 14).	bind
49473	1	11140	7	10	NULL	NULL	NULL	 aggrecan	GP		bind					hyaluronan	GP				NULL	bovine cartilage explants	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_9_6321_s_23	10692431	A more recent study demonstrated that the extent of tissue compression, with the concomitant changes in proteoglycan concentration and pH of the extracellular matrix, could influence the hyaluronan binding properties of aggrecan in bovine cartilage explants ( 14).	bind
50307	2	11140	7	10	NULL	NULL	NULL	proteoglycan	GP	change in concentration of	influence					statement 1	Process				NULL	bovine cartilage explants	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_9_6321_s_23	10692431	A more recent study demonstrated that the extent of tissue compression, with the concomitant changes in proteoglycan concentration and pH of the extracellular matrix, could influence the hyaluronan binding properties of aggrecan in bovine cartilage explants ( 14).	bind
50308	3	11140	7	10	NULL	NULL	NULL	extracellular matrix	CellComponent	change in pH of	influence					statement 1	Process				NULL	bovine cartilage explants	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_9_6321_s_23	10692431	A more recent study demonstrated that the extent of tissue compression, with the concomitant changes in proteoglycan concentration and pH of the extracellular matrix, could influence the hyaluronan binding properties of aggrecan in bovine cartilage explants ( 14).	bind
43234	1	11141	6	10	NULL	NULL	NULL	SDF-1	GP		in complex with					CXCR4 receptor	GP				NULL	surface of HeLa cells in vitro	NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
44278	2	11141	6	10	NULL	NULL	NULL	SDF-1	GP		in complex with					CXCR4 receptor	GP				NULL	primary lymphocytes in vitro	NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
44279	3	11141	6	10	NULL	NULL	NULL	SDF-1	GP		in complex with					CXCR4 receptor	GP				NULL	macrophages in vitro \t	NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
44976	4	11141	6	10	NULL	NULL	NULL	syndecan-4	GP		bind					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
44977	5	11141	6	10	NULL	NULL	NULL	syndecan-4	GP		bind					statement 2	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
44978	6	11141	6	10	NULL	NULL	NULL	syndecan-4	GP		bind					statement 3	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
44979	7	11141	6	10	NULL	NULL	NULL	syndecan-1	GP		does not bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
44980	8	11141	6	10	NULL	NULL	NULL	syndecan-1	GP		does not bind					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
44981	9	11141	6	10	NULL	NULL	NULL	syndecan-1	GP		does not bind					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
44982	10	11141	6	10	NULL	NULL	NULL	syndecan-2	GP		does not bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
44983	11	11141	6	10	NULL	NULL	NULL	syndecan-2	GP		does not bind					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
44984	12	11141	6	10	NULL	NULL	NULL	syndecan-2	GP		does not bind					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
44985	13	11141	6	10	NULL	NULL	NULL	betaglycan	GP		does not bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
67700	14	11141	6	10	NULL	0	NULL	betaglycan	GP		does not bind					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
67701	15	11141	6	10	NULL	0	NULL	betaglycan	GP		does not bind					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
67703	16	11141	6	10	NULL	0	NULL	CD44	GP		does not bind					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
67704	17	11141	6	10	NULL	0	NULL	CD44	GP		does not bind					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
67705	18	11141	6	10	NULL	0	NULL	CD44	GP		does not bind					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
49474	1	11141	7	10	NULL	NULL	NULL	SDF-1	GP		in complex with					CXCR4 receptor	GP				NULL	surface of HeLa cells in vitro	NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
49475	2	11141	7	10	NULL	NULL	NULL	 SDF-1	GP		in complex with					CXCR4 receptor 	GP				NULL	primary lymphocytes in vitro	NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
49476	3	11141	7	10	NULL	NULL	NULL	SDF-1	GP		in complex with					CXCR4 receptor	GP				NULL	macrophages in vitro	NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
49477	4	11141	7	10	NULL	NULL	NULL	syndecan-4	GP		bind					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
49478	5	11141	7	10	NULL	NULL	NULL	syndecan-4	GP		bind					statement 2	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
49479	6	11141	7	10	NULL	NULL	NULL	syndecan-4	GP		bind					statement 3	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
49480	7	11141	7	10	NULL	NULL	NULL	syndecan-1	GP		does not bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
49481	8	11141	7	10	NULL	NULL	NULL	syndecan-1	GP		does not bind					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
49482	9	11141	7	10	NULL	NULL	NULL	syndecan-1	GP		does not bind					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
49483	10	11141	7	10	NULL	NULL	NULL	syndecan-2	GP		does not bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
49484	11	11141	7	10	NULL	NULL	NULL	syndecan-2	GP		does not bind					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
49485	12	11141	7	10	NULL	NULL	NULL	syndecan-2	GP		does not bind					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
49486	13	11141	7	10	NULL	NULL	NULL	betaglycan	GP		does not bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
49487	14	11141	7	10	NULL	NULL	NULL	betaglycan	GP		does not bind					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
49488	15	11141	7	10	NULL	NULL	NULL	betaglycan	GP		does not bind					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
49489	16	11141	7	10	NULL	NULL	NULL	CD44	GP		does not bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
49490	17	11141	7	10	NULL	NULL	NULL	CD44	GP		does not bind					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
49491	18	11141	7	10	NULL	NULL	NULL	CD44	GP		does not bind					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_282_1_152_s_208	15936336	A more recent study has shown that syndecan-4 binds SDF-1 in a complex with the  CXCR4 receptor on the surface of HeLa cells, as well as on primary lymphocytes and  macrophages in vitro, while syndecan-1, syndecan-2, betaglycan, and CD44 did not  (  Hamon et al., 2004).	bind
43235	1	11142	6	10	NULL	NULL	NULL	heparin	GP		bind					HSV-1	Organism				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_24850_s_34	9312084	A more recent study implicated a variety of sulfate groups in the binding of heparin to HSV-1 ( 13).	bind
43236	2	11142	6	10	NULL	NULL	NULL	sulfate groups	Chemical		plays a role in					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_24850_s_34	9312084	A more recent study implicated a variety of sulfate groups in the binding of heparin to HSV-1 ( 13).	bind
49492	1	11142	7	10	NULL	NULL	NULL	heparin	GP		bind					HSV-1	Organism				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_24850_s_34	9312084	A more recent study implicated a variety of sulfate groups in the binding of heparin to HSV-1 ( 13).	bind
49493	2	11142	7	10	NULL	NULL	NULL	sulfate groups	Chemical		is implicated in					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_24850_s_34	9312084	A more recent study implicated a variety of sulfate groups in the binding of heparin to HSV-1 ( 13).	bind
43237	1	11143	6	10	NULL	NULL	NULL	Sp1	GP		bind					Hmga2 gene	GP	proximal		promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_6_2296_s_307	14993269	A more recent study of the transcriptional inhibition of the  Hmga2 gene following TSA treatment has suggested that repression results from a decrease in Sp1 and Sp3 binding to the proximal promoter ( ).	bind
43238	2	11143	6	10	NULL	NULL	NULL	Sp3	GP		bind					Hmga2 gene	GP	proximal		promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_6_2296_s_307	14993269	A more recent study of the transcriptional inhibition of the  Hmga2 gene following TSA treatment has suggested that repression results from a decrease in Sp1 and Sp3 binding to the proximal promoter ( ).	bind
43239	3	11143	6	10	NULL	NULL	NULL	TSA	Chemical	treatment	inhibits					Hmga2 gene	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_6_2296_s_307	14993269	A more recent study of the transcriptional inhibition of the  Hmga2 gene following TSA treatment has suggested that repression results from a decrease in Sp1 and Sp3 binding to the proximal promoter ( ).	bind
43240	4	11143	6	10	NULL	NULL	NULL	statement 3	Process		occurs due to					statement 1	Process	decrease in			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_6_2296_s_307	14993269	A more recent study of the transcriptional inhibition of the  Hmga2 gene following TSA treatment has suggested that repression results from a decrease in Sp1 and Sp3 binding to the proximal promoter ( ).	bind
43241	5	11143	6	10	NULL	NULL	NULL	statement 3	Process		occurs due to					statement 2	Process	decrease in			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_6_2296_s_307	14993269	A more recent study of the transcriptional inhibition of the  Hmga2 gene following TSA treatment has suggested that repression results from a decrease in Sp1 and Sp3 binding to the proximal promoter ( ).	bind
49494	1	11143	7	10	NULL	NULL	NULL	Sp1	GP		bind					 Hmga2 gene	GP	proximal		promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_6_2296_s_307	14993269	A more recent study of the transcriptional inhibition of the  Hmga2 gene following TSA treatment has suggested that repression results from a decrease in Sp1 and Sp3 binding to the proximal promoter ( ).	bind
49495	2	11143	7	10	NULL	NULL	NULL	Sp3	GP		bind					Hmga2 gene	GP	proximal		promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_6_2296_s_307	14993269	A more recent study of the transcriptional inhibition of the  Hmga2 gene following TSA treatment has suggested that repression results from a decrease in Sp1 and Sp3 binding to the proximal promoter ( ).	bind
49496	4	11143	7	10	NULL	NULL	NULL	statement 3	Process	decrease in	results in					statement 1	Process	decrease in			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_6_2296_s_307	14993269	A more recent study of the transcriptional inhibition of the  Hmga2 gene following TSA treatment has suggested that repression results from a decrease in Sp1 and Sp3 binding to the proximal promoter ( ).	bind
50309	3	11143	7	10	NULL	NULL	NULL	TSA	Chemical	treatment	inhibits					Hmga2 gene	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_6_2296_s_307	14993269	A more recent study of the transcriptional inhibition of the  Hmga2 gene following TSA treatment has suggested that repression results from a decrease in Sp1 and Sp3 binding to the proximal promoter ( ).	bind
43242	1	11144	6	10	NULL	NULL	NULL	ERalpha	GP		does not bind					DR1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_135	11452016	A more recent study showed that neither ERalpha nor ERbeta bound to DR1 or DR4, irrespective of the presence or absence of RXR ( 122).	bind
43243	2	11144	6	10	NULL	NULL	NULL	ERalpha	GP		does not bind					DR4	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_135	11452016	A more recent study showed that neither ERalpha nor ERbeta bound to DR1 or DR4, irrespective of the presence or absence of RXR ( 122).	bind
43244	3	11144	6	10	NULL	NULL	NULL	ERbeta	GP		does not bind					DR1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_135	11452016	A more recent study showed that neither ERalpha nor ERbeta bound to DR1 or DR4, irrespective of the presence or absence of RXR ( 122).	bind
43245	4	11144	6	10	NULL	NULL	NULL	ERbeta	GP		does not bind					DR4	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_135	11452016	A more recent study showed that neither ERalpha nor ERbeta bound to DR1 or DR4, irrespective of the presence or absence of RXR ( 122).	bind
49498	1	11144	7	10	NULL	NULL	NULL	ERalpha	GP		does not bind					DR1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_135	11452016	A more recent study showed that neither ERalpha nor ERbeta bound to DR1 or DR4, irrespective of the presence or absence of RXR ( 122).	bind
49499	2	11144	7	10	NULL	NULL	NULL	ERalpha	GP		does not bind					DR4	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_135	11452016	A more recent study showed that neither ERalpha nor ERbeta bound to DR1 or DR4, irrespective of the presence or absence of RXR ( 122).	bind
49500	3	11144	7	10	NULL	NULL	NULL	ERbeta	GP		does not bind					DR1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_135	11452016	A more recent study showed that neither ERalpha nor ERbeta bound to DR1 or DR4, irrespective of the presence or absence of RXR ( 122).	bind
49501	4	11144	7	10	NULL	NULL	NULL	ERbeta	GP		does not bind					DR4	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_2905_s_135	11452016	A more recent study showed that neither ERalpha nor ERbeta bound to DR1 or DR4, irrespective of the presence or absence of RXR ( 122).	bind
43246	1	11145	6	10	NULL	NULL	NULL	p53	GP	mutant	bind			core domain		p73	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_21_18817_s_330	11893750	A more recent work has reported that the core domain of mutant p53 can either bind to p73 or to p63 ( 42).	bind
43247	2	11145	6	10	NULL	NULL	NULL	p53	GP	mutant	bind			core domain		p63	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_21_18817_s_330	11893750	A more recent work has reported that the core domain of mutant p53 can either bind to p73 or to p63 ( 42).	bind
43248	3	11145	6	10	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_21_18817_s_330	11893750	A more recent work has reported that the core domain of mutant p53 can either bind to p73 or to p63 ( 42).	bind
49502	1	11145	7	10	NULL	NULL	NULL	p53	GP	mutant	bind 			core domain		p73	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_21_18817_s_330	11893750	A more recent work has reported that the core domain of mutant p53 can either bind to p73 or to p63 ( 42).	bind
49503	2	11145	7	10	NULL	NULL	NULL	p53	GP	mutant	bind			core domain		p63	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_21_18817_s_330	11893750	A more recent work has reported that the core domain of mutant p53 can either bind to p73 or to p63 ( 42).	bind
49504	3	11145	7	10	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_21_18817_s_330	11893750	A more recent work has reported that the core domain of mutant p53 can either bind to p73 or to p63 ( 42).	bind
43249	1	11146	6	10	NULL	NULL	NULL	B2	GP		bind					E2	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_gene_305_2_205_s_210	12609741	A more rigorous examination of the sequence recognition characteristics of human Sp1 compared to B2 was performed by mutating critical nucleotides known to be important for B2 binding to E2.	bind
49505	1	11146	7	10	NULL	NULL	NULL	 B2	GP		bind					E2	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_gene_305_2_205_s_210	12609741	A more rigorous examination of the sequence recognition characteristics of human Sp1 compared to B2 was performed by mutating critical nucleotides known to be important for B2 binding to E2.	bind
43250	1	11147	6	10	NULL	NULL	NULL	tubulin	GP		bind					stathmin	GP		N-terminal extension of the core		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_10_6841_s_259	10702243	A more seducing hypothesis could be that tubulin binding to stathmin may occur in two different ways, an "`N way"` and a "`C way,"` in which either an N- or a C-terminal extension of the core would allow binding of stathmin to tubulin.	bind
50310	2	11147	6	10	NULL	NULL	NULL	tubulin	GP		bind					stathmin	GP		C-terminal extension of the core		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_10_6841_s_259	10702243	A more seducing hypothesis could be that tubulin binding to stathmin may occur in two different ways, an "`N way"` and a "`C way,"` in which either an N- or a C-terminal extension of the core would allow binding of stathmin to tubulin.	bind
49506	1	11147	7	10	NULL	NULL	NULL	tubulin	GP		bind					stathmin	GP		N-terminal extension of the core		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_10_6841_s_259	10702243	A more seducing hypothesis could be that tubulin binding to stathmin may occur in two different ways, an "`N way"` and a "`C way,"` in which either an N- or a C-terminal extension of the core would allow binding of stathmin to tubulin.	bind
49507	2	11147	7	10	NULL	NULL	NULL	tubulin 	GP		bind					stathmin	GP		C-terminal extension of the core		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_10_6841_s_259	10702243	A more seducing hypothesis could be that tubulin binding to stathmin may occur in two different ways, an "`N way"` and a "`C way,"` in which either an N- or a C-terminal extension of the core would allow binding of stathmin to tubulin.	bind
43251	1	11148	6	10	NULL	NULL	NULL	UmuD``C	GP		bind					M13 DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_18_10767_s_185	8631887	A more sensitive measurement for  the binding of UmuD``C to M13 DNA was performed using fluorescence  depolarization, see  e.g. Refs.	bind
49508	1	11148	7	10	NULL	NULL	NULL	UmuD``C	GP		bind					M13 DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_18_10767_s_185	8631887	A more sensitive measurement for  the binding of UmuD``C to M13 DNA was performed using fluorescence  depolarization, see  e.g. Refs.	bind
43252	1	11149	6	10	NULL	NULL	NULL	NGF	GP		bind					TrkA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_16_24_7950_s_215	8987823	A more slowly migrating band represents NGF bound to TrkA in an undefined oligomeric complex.	bind
49509	1	11149	7	10	NULL	NULL	NULL	NGF	GP		bind					TrkA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_16_24_7950_s_215	8987823	A more slowly migrating band represents NGF bound to TrkA in an undefined oligomeric complex.	bind
43342	1	11150	6	10	NULL	NULL	NULL	HIF-1	GP		is					hypoxia-inducible factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_3_329_s_204	10024307	A more specific mechanism of hypoxia-induced gene expression might involve the transcription factor hypoxia-inducible factor or HIF-1, which binds to identified hypoxia-sensitive elements in the promoter of several hypoxia-inducible genes.	bind
43343	2	11150	6	10	NULL	NULL	NULL	HIF-1	GP		bind					hypoxia-inducible genes	GP			hypoxia-sensitive element of promoter	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_3_329_s_204	10024307	A more specific mechanism of hypoxia-induced gene expression might involve the transcription factor hypoxia-inducible factor or HIF-1, which binds to identified hypoxia-sensitive elements in the promoter of several hypoxia-inducible genes.	bind
50311	3	11150	6	10	NULL	NULL	NULL	HIF-1	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_3_329_s_204	10024307	A more specific mechanism of hypoxia-induced gene expression might involve the transcription factor hypoxia-inducible factor or HIF-1, which binds to identified hypoxia-sensitive elements in the promoter of several hypoxia-inducible genes.	bind
49511	1	11150	7	10	NULL	NULL	NULL	 HIF-1	GP		bind					hypoxia-inducible genes	GP			hypoxia-sensitive elements in the promoter	NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_3_329_s_204	10024307	A more specific mechanism of hypoxia-induced gene expression might involve the transcription factor hypoxia-inducible factor or HIF-1, which binds to identified hypoxia-sensitive elements in the promoter of several hypoxia-inducible genes.	bind
49512	2	11150	7	10	NULL	NULL	NULL	HIF-1	GP		is					hypoxia-inducible factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_3_329_s_204	10024307	A more specific mechanism of hypoxia-induced gene expression might involve the transcription factor hypoxia-inducible factor or HIF-1, which binds to identified hypoxia-sensitive elements in the promoter of several hypoxia-inducible genes.	bind
49513	3	11150	7	10	NULL	NULL	NULL	HIF-1	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_84_3_329_s_204	10024307	A more specific mechanism of hypoxia-induced gene expression might involve the transcription factor hypoxia-inducible factor or HIF-1, which binds to identified hypoxia-sensitive elements in the promoter of several hypoxia-inducible genes.	bind
43253	1	11152	6	10	NULL	NULL	NULL	PFA	Chemical		bind					RT	GP		catalytic site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_38_27744_s_229	16829515	A more suitable explanation would be that PFA and the incoming dNTP bind to the catalytic site of RT but to different mechanistic forms of the enzyme in such a way that they do not compete with each other ( ).	bind
43254	2	11152	6	10	NULL	NULL	NULL	dNTP	Chemical		bind					RT	GP		catalytic site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_38_27744_s_229	16829515	A more suitable explanation would be that PFA and the incoming dNTP bind to the catalytic site of RT but to different mechanistic forms of the enzyme in such a way that they do not compete with each other ( ).	bind
51519	3	11152	6	10	NULL	NULL	NULL	statement 1	Process		does not compete with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_38_27744_s_229	16829515	A more suitable explanation would be that PFA and the incoming dNTP bind to the catalytic site of RT but to different mechanistic forms of the enzyme in such a way that they do not compete with each other ( ).	bind
49566	1	11152	7	10	NULL	NULL	NULL	PFA 	Chemical		bind					RT	GP		catalytic site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_38_27744_s_229	16829515	A more suitable explanation would be that PFA and the incoming dNTP bind to the catalytic site of RT but to different mechanistic forms of the enzyme in such a way that they do not compete with each other ( ).	bind
49567	2	11152	7	10	NULL	NULL	NULL	dNTP	Chemical		bind					RT	GP		catalytic site		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_38_27744_s_229	16829515	A more suitable explanation would be that PFA and the incoming dNTP bind to the catalytic site of RT but to different mechanistic forms of the enzyme in such a way that they do not compete with each other ( ).	bind
49568	3	11152	7	10	NULL	NULL	NULL	statement 1	Process		does not compete with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_38_27744_s_229	16829515	A more suitable explanation would be that PFA and the incoming dNTP bind to the catalytic site of RT but to different mechanistic forms of the enzyme in such a way that they do not compete with each other ( ).	bind
44280	1	11153	6	10	NULL	NULL	NULL	amphiphysin	GP		bind					clathrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_285_5425_215_s_218	10398591	A motif L(L or I)(D, E, or N)(L or F)(D or E) (21) in the beta subunits of APs, the nonvisual arrestins, and amphiphysin (which also binds clathrin) is likely to account for the ability of these different proteins to bind clathrin.	bind
44281	2	11153	6	NULL	NULL	0	NULL	APs	NULL		is a type of	NULL				nonvisual arrestin	NULL				NULL		0	NULL	NULL	NULL	gw60_science_285_5425_215_s_218	10398591	A motif L(L or I)(D, E, or N)(L or F)(D or E) (21) in the beta subunits of APs, the nonvisual arrestins, and amphiphysin (which also binds clathrin) is likely to account for the ability of these different proteins to bind clathrin.	bind
44282	3	11153	6	NULL	NULL	0	NULL	APs	NULL		bind	NULL				clathrin	NULL				NULL		0	NULL	NULL	NULL	gw60_science_285_5425_215_s_218	10398591	A motif L(L or I)(D, E, or N)(L or F)(D or E) (21) in the beta subunits of APs, the nonvisual arrestins, and amphiphysin (which also binds clathrin) is likely to account for the ability of these different proteins to bind clathrin.	bind
44283	4	11153	6	NULL	NULL	0	NULL	amphiphysin	NULL		plays a role in	NULL		motif L in the beta subunit		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_science_285_5425_215_s_218	10398591	A motif L(L or I)(D, E, or N)(L or F)(D or E) (21) in the beta subunits of APs, the nonvisual arrestins, and amphiphysin (which also binds clathrin) is likely to account for the ability of these different proteins to bind clathrin.	bind
44284	5	11153	6	NULL	NULL	0	NULL	APs	NULL		plays a role in	NULL		motif L in the beta subunit		statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_science_285_5425_215_s_218	10398591	A motif L(L or I)(D, E, or N)(L or F)(D or E) (21) in the beta subunits of APs, the nonvisual arrestins, and amphiphysin (which also binds clathrin) is likely to account for the ability of these different proteins to bind clathrin.	bind
49569	1	11153	7	NULL	NULL	0	NULL	 APs	NULL		bind	NULL				clathrin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_science_285_5425_215_s_218	10398591	A motif L(L or I)(D, E, or N)(L or F)(D or E) (21) in the beta subunits of APs, the nonvisual arrestins, and amphiphysin (which also binds clathrin) is likely to account for the ability of these different proteins to bind clathrin.	bind
49570	2	11153	7	NULL	NULL	0	NULL	 amphiphysin	NULL		bind	NULL				clathrin	NULL				NULL		0	NULL	NULL	NULL	gw60_science_285_5425_215_s_218	10398591	A motif L(L or I)(D, E, or N)(L or F)(D or E) (21) in the beta subunits of APs, the nonvisual arrestins, and amphiphysin (which also binds clathrin) is likely to account for the ability of these different proteins to bind clathrin.	bind
49571	3	11153	7	NULL	NULL	0	NULL	APs	NULL		is responsible for	NULL		motif L  in the beta subunits 		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_science_285_5425_215_s_218	10398591	A motif L(L or I)(D, E, or N)(L or F)(D or E) (21) in the beta subunits of APs, the nonvisual arrestins, and amphiphysin (which also binds clathrin) is likely to account for the ability of these different proteins to bind clathrin.	bind
49572	4	11153	7	NULL	NULL	0	NULL	APs	NULL		is required for	NULL		motifs I in the beta subunit		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_science_285_5425_215_s_218	10398591	A motif L(L or I)(D, E, or N)(L or F)(D or E) (21) in the beta subunits of APs, the nonvisual arrestins, and amphiphysin (which also binds clathrin) is likely to account for the ability of these different proteins to bind clathrin.	bind
49573	5	11153	7	NULL	NULL	0	NULL	statement 3	NULL		is an alternative to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_science_285_5425_215_s_218	10398591	A motif L(L or I)(D, E, or N)(L or F)(D or E) (21) in the beta subunits of APs, the nonvisual arrestins, and amphiphysin (which also binds clathrin) is likely to account for the ability of these different proteins to bind clathrin.	bind
49574	6	11153	7	NULL	NULL	0	NULL	APs	NULL		is required for	NULL		motif D in the beta subunits		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_science_285_5425_215_s_218	10398591	A motif L(L or I)(D, E, or N)(L or F)(D or E) (21) in the beta subunits of APs, the nonvisual arrestins, and amphiphysin (which also binds clathrin) is likely to account for the ability of these different proteins to bind clathrin.	bind
49575	7	11153	7	NULL	NULL	0	NULL	APs	NULL		is required for	NULL		motif E in the beta subunit		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_science_285_5425_215_s_218	10398591	A motif L(L or I)(D, E, or N)(L or F)(D or E) (21) in the beta subunits of APs, the nonvisual arrestins, and amphiphysin (which also binds clathrin) is likely to account for the ability of these different proteins to bind clathrin.	bind
49576	8	11153	7	NULL	NULL	0	NULL	AP	NULL		is required for	NULL		motif N in the beta subunit		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_science_285_5425_215_s_218	10398591	A motif L(L or I)(D, E, or N)(L or F)(D or E) (21) in the beta subunits of APs, the nonvisual arrestins, and amphiphysin (which also binds clathrin) is likely to account for the ability of these different proteins to bind clathrin.	bind
49577	9	11153	7	NULL	NULL	0	NULL	statement 6	NULL		is an alternative to	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw60_science_285_5425_215_s_218	10398591	A motif L(L or I)(D, E, or N)(L or F)(D or E) (21) in the beta subunits of APs, the nonvisual arrestins, and amphiphysin (which also binds clathrin) is likely to account for the ability of these different proteins to bind clathrin.	bind
49578	10	11153	7	NULL	NULL	0	NULL	statement 7	NULL		is an alternative to	NULL				statement 8	NULL				NULL		0	NULL	NULL	NULL	gw60_science_285_5425_215_s_218	10398591	A motif L(L or I)(D, E, or N)(L or F)(D or E) (21) in the beta subunits of APs, the nonvisual arrestins, and amphiphysin (which also binds clathrin) is likely to account for the ability of these different proteins to bind clathrin.	bind
49579	11	11153	7	10	NULL	0	NULL	APs	NULL		is a type of	NULL				nonvisual arrestins	NULL				NULL		NULL	NULL	NULL	NULL	gw60_science_285_5425_215_s_218	10398591	A motif L(L or I)(D, E, or N)(L or F)(D or E) (21) in the beta subunits of APs, the nonvisual arrestins, and amphiphysin (which also binds clathrin) is likely to account for the ability of these different proteins to bind clathrin.	bind
49581	13	11153	7	NULL	NULL	0	NULL	APs	NULL		is required for	NULL		motif F in the beta subunit		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_science_285_5425_215_s_218	10398591	A motif L(L or I)(D, E, or N)(L or F)(D or E) (21) in the beta subunits of APs, the nonvisual arrestins, and amphiphysin (which also binds clathrin) is likely to account for the ability of these different proteins to bind clathrin.	bind
49582	14	11153	7	NULL	NULL	0	NULL	statement 3	NULL		is an alternative to	NULL				statement 13	NULL				NULL		0	NULL	NULL	NULL	gw60_science_285_5425_215_s_218	10398591	A motif L(L or I)(D, E, or N)(L or F)(D or E) (21) in the beta subunits of APs, the nonvisual arrestins, and amphiphysin (which also binds clathrin) is likely to account for the ability of these different proteins to bind clathrin.	bind
43271	1	11154	6	10	NULL	NULL	NULL	E2F-1	GP		bind			\tY(X7)E(X3)DLF motif		Rb	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6520_s_288	12944478	A motif with a similar format, described as Y(X7)E(X3)DLF, has been proposed to be involved in the binding of E2F-1 and NF-IL-6 (C/EBPbeta) to Rb ( 8).	bind
43272	2	11154	6	10	NULL	NULL	NULL	NF-IL-6 (C/EBPbeta)	GP		bind			\tY(X7)E(X3)DLF motif		Rb	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6520_s_288	12944478	A motif with a similar format, described as Y(X7)E(X3)DLF, has been proposed to be involved in the binding of E2F-1 and NF-IL-6 (C/EBPbeta) to Rb ( 8).	bind
49585	1	11154	7	10	NULL	NULL	NULL	E2F-1 	GP		bind			\tY(X7)E(X3)DLF motif		Rb	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6520_s_288	12944478	A motif with a similar format, described as Y(X7)E(X3)DLF, has been proposed to be involved in the binding of E2F-1 and NF-IL-6 (C/EBPbeta) to Rb ( 8).	bind
49586	2	11154	7	10	NULL	NULL	NULL	NF-IL-6 (C/EBPbeta)	GP		bind			\tY(X7)E(X3)DLF motif		Rb	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_18_6520_s_288	12944478	A motif with a similar format, described as Y(X7)E(X3)DLF, has been proposed to be involved in the binding of E2F-1 and NF-IL-6 (C/EBPbeta) to Rb ( 8).	bind
43274	1	11155	6	10	NULL	NULL	NULL	Cdk complex	GP		contains					cyclins A	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7488_s_299	14559997	A motif within the N terminus of Cdc25A confers binding of Cdc25A to Cdk complexes containing cyclins A and E but not B1 ( ).	bind
43275	2	11155	6	10	NULL	NULL	NULL	Cdk complex	GP		contains					cyclin E	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7488_s_299	14559997	A motif within the N terminus of Cdc25A confers binding of Cdc25A to Cdk complexes containing cyclins A and E but not B1 ( ).	bind
43276	3	11155	6	10	NULL	NULL	NULL	Cdk complex	GP		contain					cyclin B1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7488_s_299	14559997	A motif within the N terminus of Cdc25A confers binding of Cdc25A to Cdk complexes containing cyclins A and E but not B1 ( ).	bind
43695	4	11155	6	10	NULL	NULL	NULL	Cdc25A	GP		bind			motif within N terminus		statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7488_s_299	14559997	A motif within the N terminus of Cdc25A confers binding of Cdc25A to Cdk complexes containing cyclins A and E but not B1 ( ).	bind
43698	5	11155	6	10	NULL	NULL	NULL	Cdc25A	GP		bind			motif within N terminus		statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7488_s_299	14559997	A motif within the N terminus of Cdc25A confers binding of Cdc25A to Cdk complexes containing cyclins A and E but not B1 ( ).	bind
51520	6	11155	6	10	NULL	NULL	NULL	Cdc25A	GP		does not bind			motif within N terminus		statement 3	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7488_s_299	14559997	A motif within the N terminus of Cdc25A confers binding of Cdc25A to Cdk complexes containing cyclins A and E but not B1 ( ).	bind
49593	1	11155	7	10	NULL	NULL	NULL	Cdk complex	GP		contains					cyclins A	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7488_s_299	14559997	A motif within the N terminus of Cdc25A confers binding of Cdc25A to Cdk complexes containing cyclins A and E but not B1 ( ).	bind
49594	2	11155	7	10	NULL	NULL	NULL	Cdk complex	GP		contains					cyclins E	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7488_s_299	14559997	A motif within the N terminus of Cdc25A confers binding of Cdc25A to Cdk complexes containing cyclins A and E but not B1 ( ).	bind
49596	3	11155	7	10	NULL	NULL	NULL	Cdk complex	GP		contains					cyclin B1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7488_s_299	14559997	A motif within the N terminus of Cdc25A confers binding of Cdc25A to Cdk complexes containing cyclins A and E but not B1 ( ).	bind
49597	4	11155	7	10	NULL	NULL	NULL	Cdc25A	GP		bind			motif within the N terminus		statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7488_s_299	14559997	A motif within the N terminus of Cdc25A confers binding of Cdc25A to Cdk complexes containing cyclins A and E but not B1 ( ).	bind
49599	5	11155	7	10	NULL	NULL	NULL	Cdc25A	GP		bind			motif within the N terminus		statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7488_s_299	14559997	A motif within the N terminus of Cdc25A confers binding of Cdc25A to Cdk complexes containing cyclins A and E but not B1 ( ).	bind
49600	6	11155	7	10	NULL	NULL	NULL	Cdc25A	GP		does not bind			motif within the N terminus		statement 3	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_21_7488_s_299	14559997	A motif within the N terminus of Cdc25A confers binding of Cdc25A to Cdk complexes containing cyclins A and E but not B1 ( ).	bind
43700	1	11157	6	10	NULL	NULL	NULL	fVII	GP	mouse	bind		tightly	targeting domain		tissue factor	GP	human			NULL	tumor cells	NULL	NULL	NULL	NULL	gw60_pnas_97_16_9221_s_155	10922073	A mouse fVII targeting domain was used for the experiments involving human tumor xenografts growing in SCID mice, because it binds tightly both to human tissue factor on the tumor cells and to mouse tissue factor on the mouse endothelial cells in the tumor vasculature.	bind
44287	2	11157	6	10	NULL	NULL	NULL	fVII	GP	mouse	bind		tightly	targeting domain		tissue factor	GP	mouse			NULL	mouse endothelial cells in the tumor vasculature	NULL	NULL	NULL	NULL	gw60_pnas_97_16_9221_s_155	10922073	A mouse fVII targeting domain was used for the experiments involving human tumor xenografts growing in SCID mice, because it binds tightly both to human tissue factor on the tumor cells and to mouse tissue factor on the mouse endothelial cells in the tumor vasculature.	bind
49601	1	11157	7	10	NULL	NULL	NULL	 fVII	GP	mouse	bind		tightly	targeting domain		tissue factor	GP	human			NULL	tumor cells	NULL	NULL	NULL	NULL	gw60_pnas_97_16_9221_s_155	10922073	A mouse fVII targeting domain was used for the experiments involving human tumor xenografts growing in SCID mice, because it binds tightly both to human tissue factor on the tumor cells and to mouse tissue factor on the mouse endothelial cells in the tumor vasculature.	bind
49603	2	11157	7	10	NULL	NULL	NULL	fVII	GP	mouse	bind		tightly	targeting domain		tissue factor	GP	mouse			NULL	mouse endothelial cells in the tumor vasculature	NULL	NULL	NULL	NULL	gw60_pnas_97_16_9221_s_155	10922073	A mouse fVII targeting domain was used for the experiments involving human tumor xenografts growing in SCID mice, because it binds tightly both to human tissue factor on the tumor cells and to mouse tissue factor on the mouse endothelial cells in the tumor vasculature.	bind
43707	1	11159	6	10	NULL	NULL	NULL	cGMP	Chemical		bind					PDE5	GP		GAF A domain		NULL		NULL	NULL	NULL	NULL	gw60_embo_22_3_469_s_88	12554648	A mouse monoclonal antibody specifically blocks cGMP binding to the GAF A domain of PDE5   he previous studies showed that a short pre-incubation of PDE5 with cGMP on ice did not cause PDE5 phosphorylation, but was sufficient to induce PDE5 activation.	bind
43709	2	11159	6	10	NULL	NULL	NULL	monoclonal antibody	GP	mouse	blocks		specifically			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_3_469_s_88	12554648	A mouse monoclonal antibody specifically blocks cGMP binding to the GAF A domain of PDE5   he previous studies showed that a short pre-incubation of PDE5 with cGMP on ice did not cause PDE5 phosphorylation, but was sufficient to induce PDE5 activation.	bind
49604	1	11159	7	10	NULL	NULL	NULL	cGMP	Chemical		bind					PDE5	GP		GAF A domain		NULL		NULL	NULL	NULL	NULL	gw60_embo_22_3_469_s_88	12554648	A mouse monoclonal antibody specifically blocks cGMP binding to the GAF A domain of PDE5   he previous studies showed that a short pre-incubation of PDE5 with cGMP on ice did not cause PDE5 phosphorylation, but was sufficient to induce PDE5 activation.	bind
49605	2	11159	7	10	NULL	NULL	NULL	monoclonal antibody	GP	mouse	blocks		specifically			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_22_3_469_s_88	12554648	A mouse monoclonal antibody specifically blocks cGMP binding to the GAF A domain of PDE5   he previous studies showed that a short pre-incubation of PDE5 with cGMP on ice did not cause PDE5 phosphorylation, but was sufficient to induce PDE5 activation.	bind
44288	1	11162	6	NULL	NULL	0	NULL		NULL		bind	NULL	covalently	N of Lys216		retina	NULL		C-15		NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1565_2_144_s_243	12409192	A movement of the side chain atoms may have been anticipated from the fact that N  of Lys216 (i.e. the Schiff base nitrogen) is covalently bound to C15 of the retinal ( Fig. 2A) and necessarily undergoes a significant movement in response to photoisomerization about the C13=C14 bond.	bind
51521	2	11162	6	10	NULL	NULL	NULL	N of Lys216	Chemical		is					Schiff base nitrogen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1565_2_144_s_243	12409192	A movement of the side chain atoms may have been anticipated from the fact that N  of Lys216 (i.e. the Schiff base nitrogen) is covalently bound to C15 of the retinal ( Fig. 2A) and necessarily undergoes a significant movement in response to photoisomerization about the C13=C14 bond.	bind
49606	1	11162	7	10	NULL	0	NULL		NULL		bind	NULL	covalently	N of Lys216		retinal 	NULL		C15		NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1565_2_144_s_243	12409192	A movement of the side chain atoms may have been anticipated from the fact that N  of Lys216 (i.e. the Schiff base nitrogen) is covalently bound to C15 of the retinal ( Fig. 2A) and necessarily undergoes a significant movement in response to photoisomerization about the C13=C14 bond.	bind
49607	2	11162	7	10	NULL	NULL	NULL	N of Lys216	Chemical		is					Schiff base nitrogen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1565_2_144_s_243	12409192	A movement of the side chain atoms may have been anticipated from the fact that N  of Lys216 (i.e. the Schiff base nitrogen) is covalently bound to C15 of the retinal ( Fig. 2A) and necessarily undergoes a significant movement in response to photoisomerization about the C13=C14 bond.	bind
51522	1	11163	6	10	NULL	NULL	NULL	MTase	GP		is associated with					restriction endonuclease	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_7_1491_s_270	11266551	A MTase not long ago associated with a restriction endonuclease may momentarily exist alone, before selective pressures swallow it as well.	bind
49608	1	11163	7	10	NULL	NULL	NULL	MTase	GP		is associated with					restriction endonuclease	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_7_1491_s_270	11266551	A MTase not long ago associated with a restriction endonuclease may momentarily exist alone, before selective pressures swallow it as well.	bind
43711	2	11164	6	10	NULL	NULL	NULL	TFIIIA	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_33_21352_s_172	9694896	A much different situation was found for TFIIIA binding to 5 S DNA assembled into a complete nucleosome.	bind
43712	1	11164	6	10	NULL	NULL	NULL	5S DNA	NucleicAcid		is assembled into					nucleosome	Chromosome				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_33_21352_s_172	9694896	A much different situation was found for TFIIIA binding to 5 S DNA assembled into a complete nucleosome.	bind
49609	2	11164	7	NULL	NULL	0	NULL	 TFIIIA	NULL		bind	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_33_21352_s_172	9694896	A much different situation was found for TFIIIA binding to 5 S DNA assembled into a complete nucleosome.	bind
49610	1	11164	7	10	NULL	NULL	NULL	5 S DNA	NucleicAcid		assemble into					nucleosome	Chromosome				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_33_21352_s_172	9694896	A much different situation was found for TFIIIA binding to 5 S DNA assembled into a complete nucleosome.	bind
44289	1	11165	6	10	NULL	NULL	NULL	GP63	GP	glycosylated	bind					ConA	GP	WT;;promastigotes			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_31_27968_s_185	12029085	A much higher level of glycosylated GP63 bound to ConA from WT promastigotes ( lane 1) than delta gpi8 cells ( lane 2).	bind
44290	2	11165	6	10	NULL	NULL	NULL	GP63	GP	glycosylated	bind					ConA	GP	delta gpi8 cells			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_31_27968_s_185	12029085	A much higher level of glycosylated GP63 bound to ConA from WT promastigotes ( lane 1) than delta gpi8 cells ( lane 2).	bind
44291	3	11165	6	10	NULL	NULL	NULL	statement 1	Process		is higher than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_31_27968_s_185	12029085	A much higher level of glycosylated GP63 bound to ConA from WT promastigotes ( lane 1) than delta gpi8 cells ( lane 2).	bind
49611	1	11165	7	10	NULL	NULL	NULL	GP63	GP	glycosylated	bind					ConA	GP	WT;;promastigotes			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_31_27968_s_185	12029085	A much higher level of glycosylated GP63 bound to ConA from WT promastigotes ( lane 1) than delta gpi8 cells ( lane 2).	bind
49612	2	11165	7	10	NULL	NULL	NULL	GP63	GP	glycosylated	bind					ConA	GP	 delta gpi8 cells 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_31_27968_s_185	12029085	A much higher level of glycosylated GP63 bound to ConA from WT promastigotes ( lane 1) than delta gpi8 cells ( lane 2).	bind
49613	3	11165	7	10	NULL	NULL	NULL	statement 1	Process		is higher than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_31_27968_s_185	12029085	A much higher level of glycosylated GP63 bound to ConA from WT promastigotes ( lane 1) than delta gpi8 cells ( lane 2).	bind
43713	1	11166	6	10	NULL	NULL	NULL	CDK2	GP		bind					p27	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_52_52052_s_70	14551212	A much smaller fraction of CDK2 was bound to p27.	bind
49614	1	11166	7	10	NULL	NULL	NULL	 CDK2 	GP		bind					p27	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_52_52052_s_70	14551212	A much smaller fraction of CDK2 was bound to p27.	bind
43714	1	11168	6	10	NULL	NULL	NULL	GTP	Chemical		bind					Rac	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_22_6527_s_87	9822598	A much weaker interaction was detected with the GTP-bound form of Rac, and no binding was observed with Rho.	bind
49616	1	11168	7	10	NULL	NULL	NULL	GTP	Chemical		bind					Rac	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_22_6527_s_87	9822598	A much weaker interaction was detected with the GTP-bound form of Rac, and no binding was observed with Rho.	bind
43715	1	11169	6	10	NULL	NULL	NULL	ORC	GP		is					origin recognition complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_4_3_238_s_10	7857395	A multi-protein origin recognition complex (ORC), which binds specifically to yeast replication origins, has been shown to play a key role in transcriptional silencing as well as in DNA replication      [2-6]  .	bind
43716	2	11169	6	10	NULL	NULL	NULL	ORC	GP		bind		specifically			replication origin	NucleicAcid	Yeast			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_4_3_238_s_10	7857395	A multi-protein origin recognition complex (ORC), which binds specifically to yeast replication origins, has been shown to play a key role in transcriptional silencing as well as in DNA replication      [2-6]  .	bind
43717	3	11169	6	10	NULL	NULL	NULL	statement 2	Process		plays a role in					transcription	Process	silencing of			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_4_3_238_s_10	7857395	A multi-protein origin recognition complex (ORC), which binds specifically to yeast replication origins, has been shown to play a key role in transcriptional silencing as well as in DNA replication      [2-6]  .	bind
43718	4	11169	6	10	NULL	NULL	NULL	ORC	GP		plays a role in					DNA 	NucleicAcid	replication of			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_4_3_238_s_10	7857395	A multi-protein origin recognition complex (ORC), which binds specifically to yeast replication origins, has been shown to play a key role in transcriptional silencing as well as in DNA replication      [2-6]  .	bind
49617	1	11169	7	10	NULL	NULL	NULL	ORC	GP		bind		specifically			 replication origins	NucleicAcid	yeast			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_4_3_238_s_10	7857395	A multi-protein origin recognition complex (ORC), which binds specifically to yeast replication origins, has been shown to play a key role in transcriptional silencing as well as in DNA replication      [2-6]  .	bind
49618	2	11169	7	10	NULL	NULL	NULL	statement 1	Process		play a key role in					transcription	Process	silencing of			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_4_3_238_s_10	7857395	A multi-protein origin recognition complex (ORC), which binds specifically to yeast replication origins, has been shown to play a key role in transcriptional silencing as well as in DNA replication      [2-6]  .	bind
49619	3	11169	7	10	NULL	NULL	NULL	statement 1	Process		play a key role in					DNA 	NucleicAcid	replication of			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_4_3_238_s_10	7857395	A multi-protein origin recognition complex (ORC), which binds specifically to yeast replication origins, has been shown to play a key role in transcriptional silencing as well as in DNA replication      [2-6]  .	bind
49620	4	11169	7	10	NULL	NULL	NULL	ORC	GP		is					origin recognition complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_4_3_238_s_10	7857395	A multi-protein origin recognition complex (ORC), which binds specifically to yeast replication origins, has been shown to play a key role in transcriptional silencing as well as in DNA replication      [2-6]  .	bind
43719	1	11170	6	10	NULL	NULL	NULL	CD28RC	GP		bind		cooperatively			CD28RE	NucleicAcid			TRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_1_552_s_105	9417115	A multicomponent affinity-purified complex (CD28RC) binds cooperatively to the CD28RE-TRE and makes extensive contacts with the CD28RE-TRE sequence.	bind
51523	2	11170	6	10	NULL	NULL	NULL	CD28RC	GP		is a type of					multicomponent affinity-purified complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_1_552_s_105	9417115	A multicomponent affinity-purified complex (CD28RC) binds cooperatively to the CD28RE-TRE and makes extensive contacts with the CD28RE-TRE sequence.	bind
49621	1	11170	7	10	NULL	NULL	NULL	CD28RC	GP		bind		cooperatively			CD28RE	GP			TRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_1_552_s_105	9417115	A multicomponent affinity-purified complex (CD28RC) binds cooperatively to the CD28RE-TRE and makes extensive contacts with the CD28RE-TRE sequence.	bind
49622	2	11170	7	10	NULL	NULL	NULL	statement 1	Process		contact with		extensively			CD28RE	NucleicAcid	sequence of		TRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_1_552_s_105	9417115	A multicomponent affinity-purified complex (CD28RC) binds cooperatively to the CD28RE-TRE and makes extensive contacts with the CD28RE-TRE sequence.	bind
49623	3	11170	7	10	NULL	NULL	NULL	CD28RC	GP		is a type of					multicomponent affinity-purified complex 	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_1_552_s_105	9417115	A multicomponent affinity-purified complex (CD28RC) binds cooperatively to the CD28RE-TRE and makes extensive contacts with the CD28RE-TRE sequence.	bind
43720	1	11171	6	10	NULL	NULL	NULL	cyt bo3	GP		bind					ubiquinone-2	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_25_16879_s_33	16624801	A multifrequency (9, 34, and 94 GHz) EPR study was performed with cyt  bo3 bound to ubiquinone-2 selectively labeled with 13C at either the 1- or the 4-carbonyl carbons ( ).	bind
49624	1	11171	7	10	NULL	NULL	NULL	cyt bo3	GP		bind					ubiquinone-2	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_25_16879_s_33	16624801	A multifrequency (9, 34, and 94 GHz) EPR study was performed with cyt  bo3 bound to ubiquinone-2 selectively labeled with 13C at either the 1- or the 4-carbonyl carbons ( ).	bind
43721	1	11172	6	10	NULL	NULL	NULL	Tek	GP		is required for			Tyr;; C-terminal		Grb2	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_43_30896_s_262	10521483	A multifunctional docking site, Tyr, is also present in the C-terminal tail of Tek, and this site is required for binding of Grb2 and Grb7 as well as phosphorylation of both Grb7 and p85.	bind
43722	2	11172	6	10	NULL	NULL	NULL	Tek	GP		is required for			Tyr;; C-terminal		Grb7	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_43_30896_s_262	10521483	A multifunctional docking site, Tyr, is also present in the C-terminal tail of Tek, and this site is required for binding of Grb2 and Grb7 as well as phosphorylation of both Grb7 and p85.	bind
43723	3	11172	6	10	NULL	NULL	NULL	Tek	GP		is required for			Tyr;; C-terminal		Grb7	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_43_30896_s_262	10521483	A multifunctional docking site, Tyr, is also present in the C-terminal tail of Tek, and this site is required for binding of Grb2 and Grb7 as well as phosphorylation of both Grb7 and p85.	bind
43724	4	11172	6	10	NULL	NULL	NULL	Tek	GP		is required for			Tyr;; C-terminal		p85	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_43_30896_s_262	10521483	A multifunctional docking site, Tyr, is also present in the C-terminal tail of Tek, and this site is required for binding of Grb2 and Grb7 as well as phosphorylation of both Grb7 and p85.	bind
51524	5	11172	6	10	NULL	NULL	NULL	Tek	GP		is a type of			Tyr;; C-terminal		multifunctional docking site	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_43_30896_s_262	10521483	A multifunctional docking site, Tyr, is also present in the C-terminal tail of Tek, and this site is required for binding of Grb2 and Grb7 as well as phosphorylation of both Grb7 and p85.	bind
49626	1	11172	7	10	NULL	NULL	NULL	Tek	GP		is required for			Tyr;; C-terminal		Grb2	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_43_30896_s_262	10521483	A multifunctional docking site, Tyr, is also present in the C-terminal tail of Tek, and this site is required for binding of Grb2 and Grb7 as well as phosphorylation of both Grb7 and p85.	bind
49627	2	11172	7	10	NULL	NULL	NULL	Tek	GP		is required for			Tyr;; C-terminal		Grb7	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_43_30896_s_262	10521483	A multifunctional docking site, Tyr, is also present in the C-terminal tail of Tek, and this site is required for binding of Grb2 and Grb7 as well as phosphorylation of both Grb7 and p85.	bind
49628	3	11172	7	10	NULL	NULL	NULL	Tek	GP		is required for			Tyr;; C-terminal		 Grb7	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_43_30896_s_262	10521483	A multifunctional docking site, Tyr, is also present in the C-terminal tail of Tek, and this site is required for binding of Grb2 and Grb7 as well as phosphorylation of both Grb7 and p85.	bind
49629	4	11172	7	10	NULL	NULL	NULL	Tek	GP		is required for			Tyr;; C-terminal		p85	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_43_30896_s_262	10521483	A multifunctional docking site, Tyr, is also present in the C-terminal tail of Tek, and this site is required for binding of Grb2 and Grb7 as well as phosphorylation of both Grb7 and p85.	bind
49630	5	11172	7	10	NULL	NULL	NULL	Tek	GP		is a type of			Tyr;; C-terminal		multifunctional docking site	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_43_30896_s_262	10521483	A multifunctional docking site, Tyr, is also present in the C-terminal tail of Tek, and this site is required for binding of Grb2 and Grb7 as well as phosphorylation of both Grb7 and p85.	bind
43800	1	11173	6	10	NULL	NULL	NULL	exportin 1	GP		is 					CRM1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8751_s_1	14612415	A multifunctional domain in human CRM1 (exportin 1) mediates RanBP3 binding and multimerization of human T-cell leukemia virus type 1 Rex protein.	bind
43801	2	11173	6	10	NULL	NULL	NULL	CRM1	GP	human	mediates					Rex protein	GP	multimerization of;;human T-cell leukemia virus type 1			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8751_s_1	14612415	A multifunctional domain in human CRM1 (exportin 1) mediates RanBP3 binding and multimerization of human T-cell leukemia virus type 1 Rex protein.	bind
43802	3	11173	6	10	NULL	NULL	NULL	CRM1	GP	human	mediates					RanBP3	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8751_s_1	14612415	A multifunctional domain in human CRM1 (exportin 1) mediates RanBP3 binding and multimerization of human T-cell leukemia virus type 1 Rex protein.	bind
49631	1	11173	7	10	NULL	NULL	NULL	CRM1	GP	human	mediates					RanBP3	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8751_s_1	14612415	A multifunctional domain in human CRM1 (exportin 1) mediates RanBP3 binding and multimerization of human T-cell leukemia virus type 1 Rex protein.	bind
49632	2	11173	7	10	NULL	NULL	NULL	CRM1	GP	human	mediates					Rex protein	GP	multimerization of;;human T-cell leukemia virus type 1			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8751_s_1	14612415	A multifunctional domain in human CRM1 (exportin 1) mediates RanBP3 binding and multimerization of human T-cell leukemia virus type 1 Rex protein.	bind
49633	3	11173	7	10	NULL	NULL	NULL	CRM1	GP		is 					exportin 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8751_s_1	14612415	A multifunctional domain in human CRM1 (exportin 1) mediates RanBP3 binding and multimerization of human T-cell leukemia virus type 1 Rex protein.	bind
43803	1	11174	6	10	NULL	NULL	NULL	alpha folate receptor	GP		is involved in					folate transport	Process	intracellular			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_60_6_1288_s_21	11723236	A multigene family of high-affinity folate binding proteins (FBP) designated the alpha, beta, gamma folate receptors are thought to be involved in intracellular folate transport (Wagner, 1985  ; Kane et al., 1988  ; Henderson, 1990  ; Antony, 1996  ).	bind
43804	2	11174	6	10	NULL	NULL	NULL	beta folate receptor	GP		is involved in					folate transport	Process	intracellular			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_60_6_1288_s_21	11723236	A multigene family of high-affinity folate binding proteins (FBP) designated the alpha, beta, gamma folate receptors are thought to be involved in intracellular folate transport (Wagner, 1985  ; Kane et al., 1988  ; Henderson, 1990  ; Antony, 1996  ).	bind
43805	3	11174	6	10	NULL	NULL	NULL	gamma folate receptor	GP		is involved in					folate transport	Process	intracellular			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_60_6_1288_s_21	11723236	A multigene family of high-affinity folate binding proteins (FBP) designated the alpha, beta, gamma folate receptors are thought to be involved in intracellular folate transport (Wagner, 1985  ; Kane et al., 1988  ; Henderson, 1990  ; Antony, 1996  ).	bind
43806	4	11174	6	10	NULL	NULL	NULL	alpha folate receptor	GP		is a member of					folate binding protein family	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_60_6_1288_s_21	11723236	A multigene family of high-affinity folate binding proteins (FBP) designated the alpha, beta, gamma folate receptors are thought to be involved in intracellular folate transport (Wagner, 1985  ; Kane et al., 1988  ; Henderson, 1990  ; Antony, 1996  ).	bind
43807	5	11174	6	10	NULL	NULL	NULL	FBP	GP		is					folate binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_60_6_1288_s_21	11723236	A multigene family of high-affinity folate binding proteins (FBP) designated the alpha, beta, gamma folate receptors are thought to be involved in intracellular folate transport (Wagner, 1985  ; Kane et al., 1988  ; Henderson, 1990  ; Antony, 1996  ).	bind
43808	6	11174	6	10	NULL	NULL	NULL	beta folate receptor	GP		is a member of					folate binding protein family	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_60_6_1288_s_21	11723236	A multigene family of high-affinity folate binding proteins (FBP) designated the alpha, beta, gamma folate receptors are thought to be involved in intracellular folate transport (Wagner, 1985  ; Kane et al., 1988  ; Henderson, 1990  ; Antony, 1996  ).	bind
43809	7	11174	6	10	NULL	NULL	NULL	gamma folate receptor	GP		is a member of					folate binding protein family	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_60_6_1288_s_21	11723236	A multigene family of high-affinity folate binding proteins (FBP) designated the alpha, beta, gamma folate receptors are thought to be involved in intracellular folate transport (Wagner, 1985  ; Kane et al., 1988  ; Henderson, 1990  ; Antony, 1996  ).	bind
49634	1	11174	7	10	NULL	NULL	NULL	alpha folate receptor	GP		is involved in					 folate transport 	Process	intracellular			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_60_6_1288_s_21	11723236	A multigene family of high-affinity folate binding proteins (FBP) designated the alpha, beta, gamma folate receptors are thought to be involved in intracellular folate transport (Wagner, 1985  ; Kane et al., 1988  ; Henderson, 1990  ; Antony, 1996  ).	bind
49635	2	11174	7	10	NULL	NULL	NULL	beta folate receptor	GP		is involved in					folate transport	Process	intracellular			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_60_6_1288_s_21	11723236	A multigene family of high-affinity folate binding proteins (FBP) designated the alpha, beta, gamma folate receptors are thought to be involved in intracellular folate transport (Wagner, 1985  ; Kane et al., 1988  ; Henderson, 1990  ; Antony, 1996  ).	bind
49636	3	11174	7	10	NULL	NULL	NULL	gamma folate receptor	GP		is involved in					folate transport	Process	intracellular			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_60_6_1288_s_21	11723236	A multigene family of high-affinity folate binding proteins (FBP) designated the alpha, beta, gamma folate receptors are thought to be involved in intracellular folate transport (Wagner, 1985  ; Kane et al., 1988  ; Henderson, 1990  ; Antony, 1996  ).	bind
49637	4	11174	7	10	NULL	NULL	NULL	alpha folate receptor	GP		is a member of					folate binding protein family	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_60_6_1288_s_21	11723236	A multigene family of high-affinity folate binding proteins (FBP) designated the alpha, beta, gamma folate receptors are thought to be involved in intracellular folate transport (Wagner, 1985  ; Kane et al., 1988  ; Henderson, 1990  ; Antony, 1996  ).	bind
49638	5	11174	7	10	NULL	NULL	NULL	beta folate receptor	GP		is a member of					folate binding protein family	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_60_6_1288_s_21	11723236	A multigene family of high-affinity folate binding proteins (FBP) designated the alpha, beta, gamma folate receptors are thought to be involved in intracellular folate transport (Wagner, 1985  ; Kane et al., 1988  ; Henderson, 1990  ; Antony, 1996  ).	bind
49639	6	11174	7	10	NULL	NULL	NULL	gamma folate receptor	GP		is a member of					folate binding protein family	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_60_6_1288_s_21	11723236	A multigene family of high-affinity folate binding proteins (FBP) designated the alpha, beta, gamma folate receptors are thought to be involved in intracellular folate transport (Wagner, 1985  ; Kane et al., 1988  ; Henderson, 1990  ; Antony, 1996  ).	bind
49640	7	11174	7	10	NULL	NULL	NULL	FBP	GP		is					folate binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_60_6_1288_s_21	11723236	A multigene family of high-affinity folate binding proteins (FBP) designated the alpha, beta, gamma folate receptors are thought to be involved in intracellular folate transport (Wagner, 1985  ; Kane et al., 1988  ; Henderson, 1990  ; Antony, 1996  ).	bind
43810	1	11178	6	10	NULL	NULL	NULL	Skn7p	GP		does not bind									CDRE	NULL		NULL	NULL	NULL	NULL	gw60_embo_20_13_3473_s_255	11432834	A multipurpose Skn7p DNA-binding domain    Skn7pis a transcription factor and a DNA-binding protein, and although the CDRE was sufficient for the effect of Skn7p on Crz1p-dependent transcription, we were unable to detect Skn7p or Skn7p complex binding to the CDRE.	bind
43811	2	11178	6	10	NULL	NULL	NULL	Skn7p	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_13_3473_s_255	11432834	A multipurpose Skn7p DNA-binding domain    Skn7pis a transcription factor and a DNA-binding protein, and although the CDRE was sufficient for the effect of Skn7p on Crz1p-dependent transcription, we were unable to detect Skn7p or Skn7p complex binding to the CDRE.	bind
44986	3	11178	6	10	NULL	NULL	NULL	Skn7p	GP		is a type of					DNA-binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_13_3473_s_255	11432834	A multipurpose Skn7p DNA-binding domain    Skn7pis a transcription factor and a DNA-binding protein, and although the CDRE was sufficient for the effect of Skn7p on Crz1p-dependent transcription, we were unable to detect Skn7p or Skn7p complex binding to the CDRE.	bind
44987	4	11178	6	10	NULL	NULL	NULL	transcription	Process		is dependent on					Crz1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_13_3473_s_255	11432834	A multipurpose Skn7p DNA-binding domain    Skn7pis a transcription factor and a DNA-binding protein, and although the CDRE was sufficient for the effect of Skn7p on Crz1p-dependent transcription, we were unable to detect Skn7p or Skn7p complex binding to the CDRE.	bind
51525	5	11178	6	10	NULL	NULL	NULL	Skn7p	GP		effects					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_13_3473_s_255	11432834	A multipurpose Skn7p DNA-binding domain    Skn7pis a transcription factor and a DNA-binding protein, and although the CDRE was sufficient for the effect of Skn7p on Crz1p-dependent transcription, we were unable to detect Skn7p or Skn7p complex binding to the CDRE.	bind
51526	6	11178	6	10	NULL	NULL	NULL				is sufficient for				CDRE	statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_13_3473_s_255	11432834	A multipurpose Skn7p DNA-binding domain    Skn7pis a transcription factor and a DNA-binding protein, and although the CDRE was sufficient for the effect of Skn7p on Crz1p-dependent transcription, we were unable to detect Skn7p or Skn7p complex binding to the CDRE.	bind
49642	1	11178	7	10	NULL	NULL	NULL	 Skn7p	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_13_3473_s_255	11432834	A multipurpose Skn7p DNA-binding domain    Skn7pis a transcription factor and a DNA-binding protein, and although the CDRE was sufficient for the effect of Skn7p on Crz1p-dependent transcription, we were unable to detect Skn7p or Skn7p complex binding to the CDRE.	bind
49643	2	11178	7	10	NULL	NULL	NULL	Skn7p	GP		is a type of					DNA-binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_13_3473_s_255	11432834	A multipurpose Skn7p DNA-binding domain    Skn7pis a transcription factor and a DNA-binding protein, and although the CDRE was sufficient for the effect of Skn7p on Crz1p-dependent transcription, we were unable to detect Skn7p or Skn7p complex binding to the CDRE.	bind
49644	3	11178	7	10	NULL	NULL	NULL	transcription	Process		depends on					Crz1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_13_3473_s_255	11432834	A multipurpose Skn7p DNA-binding domain    Skn7pis a transcription factor and a DNA-binding protein, and although the CDRE was sufficient for the effect of Skn7p on Crz1p-dependent transcription, we were unable to detect Skn7p or Skn7p complex binding to the CDRE.	bind
49645	4	11178	7	10	NULL	NULL	NULL	Skn7p	GP		effect					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_13_3473_s_255	11432834	A multipurpose Skn7p DNA-binding domain    Skn7pis a transcription factor and a DNA-binding protein, and although the CDRE was sufficient for the effect of Skn7p on Crz1p-dependent transcription, we were unable to detect Skn7p or Skn7p complex binding to the CDRE.	bind
49646	5	11178	7	10	NULL	NULL	NULL				is sufficient for				CDRE	statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_13_3473_s_255	11432834	A multipurpose Skn7p DNA-binding domain    Skn7pis a transcription factor and a DNA-binding protein, and although the CDRE was sufficient for the effect of Skn7p on Crz1p-dependent transcription, we were unable to detect Skn7p or Skn7p complex binding to the CDRE.	bind
51527	6	11178	7	10	NULL	NULL	NULL	Skn7p	GP		does not bind									CDRE	NULL		NULL	NULL	NULL	NULL	gw60_embo_20_13_3473_s_255	11432834	A multipurpose Skn7p DNA-binding domain    Skn7pis a transcription factor and a DNA-binding protein, and although the CDRE was sufficient for the effect of Skn7p on Crz1p-dependent transcription, we were unable to detect Skn7p or Skn7p complex binding to the CDRE.	bind
43822	1	11179	6	10	NULL	NULL	NULL	FLNa	GP		bind					actin filament	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_37_32426_s_233	16030015	A multistep model for the regulation of the actin filament-binding of FLNa by CaM.	bind
43823	2	11179	6	10	NULL	NULL	NULL	CaM	GP		regulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_37_32426_s_233	16030015	A multistep model for the regulation of the actin filament-binding of FLNa by CaM.	bind
49647	1	11179	7	10	NULL	NULL	NULL	FLNa 	GP		bind					actin filament	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_37_32426_s_233	16030015	A multistep model for the regulation of the actin filament-binding of FLNa by CaM.	bind
49648	2	11179	7	10	NULL	NULL	NULL	CaM	GP		regulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_37_32426_s_233	16030015	A multistep model for the regulation of the actin filament-binding of FLNa by CaM.	bind
43824	1	11182	6	10	NULL	NULL	NULL	JIP-1	GP	murine	bind		specifically			JNK	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_277_5326_693_s_7	9235893	A murine cytoplasmic protein that binds specifically to JNK [the JNK interacting protein-1 (JIP-1)] was characterized and cloned.	bind
43825	2	11182	6	10	NULL	NULL	NULL	JIP-1	GP		is					JNK interacting protein-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_277_5326_693_s_7	9235893	A murine cytoplasmic protein that binds specifically to JNK [the JNK interacting protein-1 (JIP-1)] was characterized and cloned.	bind
43826	3	11182	6	10	NULL	NULL	NULL	JIP-1	GP		is a type of					cytoplasmic protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_277_5326_693_s_7	9235893	A murine cytoplasmic protein that binds specifically to JNK [the JNK interacting protein-1 (JIP-1)] was characterized and cloned.	bind
49649	1	11182	7	10	NULL	NULL	NULL	JIP-1	GP	murine	bind		specifically			 JNK	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_277_5326_693_s_7	9235893	A murine cytoplasmic protein that binds specifically to JNK [the JNK interacting protein-1 (JIP-1)] was characterized and cloned.	bind
49650	2	11182	7	10	NULL	NULL	NULL	JIP-1	GP		is a type of					cytoplasmic protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_277_5326_693_s_7	9235893	A murine cytoplasmic protein that binds specifically to JNK [the JNK interacting protein-1 (JIP-1)] was characterized and cloned.	bind
49651	3	11182	7	10	NULL	NULL	NULL	JIP-1	GP		is					JNK interacting protein-1 	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_277_5326_693_s_7	9235893	A murine cytoplasmic protein that binds specifically to JNK [the JNK interacting protein-1 (JIP-1)] was characterized and cloned.	bind
44292	1	11183	6	10	NULL	NULL	NULL	leukemia cell line	Cell	murine	is resistant to					E7010	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_jpn-j-cancer-res_92_7_11473728_s_6	11473728	A murine leukemia  cell line resistant to a sulfonamide antimitotic agent, E7010, which binds  to colchicine-binding sites on tubulin, was cross-resistant to the in  vitro growth-inhibitory effect of AM compounds.	bind
44293	2	11183	6	10	NULL	NULL	NULL	E7010	Chemical		is a type of					sulfonamide antimitotic agent	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_jpn-j-cancer-res_92_7_11473728_s_6	11473728	A murine leukemia  cell line resistant to a sulfonamide antimitotic agent, E7010, which binds  to colchicine-binding sites on tubulin, was cross-resistant to the in  vitro growth-inhibitory effect of AM compounds.	bind
44294	3	11183	6	10	NULL	NULL	NULL	leukemia cell line	Cell	murine	bind					tubulin	GP		colchicine binding site		NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_jpn-j-cancer-res_92_7_11473728_s_6	11473728	A murine leukemia  cell line resistant to a sulfonamide antimitotic agent, E7010, which binds  to colchicine-binding sites on tubulin, was cross-resistant to the in  vitro growth-inhibitory effect of AM compounds.	bind
44295	4	11183	6	10	NULL	NULL	NULL	AM compounds	Chemical		inhibits					growth	Process				NULL	in vitro	NULL	NULL	NULL	NULL	abs-batch0650-0679_jpn-j-cancer-res_92_7_11473728_s_6	11473728	A murine leukemia  cell line resistant to a sulfonamide antimitotic agent, E7010, which binds  to colchicine-binding sites on tubulin, was cross-resistant to the in  vitro growth-inhibitory effect of AM compounds.	bind
44296	5	11183	6	10	NULL	NULL	NULL	leukemia cell line	Cell	murine	is cross-resistant to					statement 4	Process				NULL	in vitro	NULL	NULL	NULL	NULL	abs-batch0650-0679_jpn-j-cancer-res_92_7_11473728_s_6	11473728	A murine leukemia  cell line resistant to a sulfonamide antimitotic agent, E7010, which binds  to colchicine-binding sites on tubulin, was cross-resistant to the in  vitro growth-inhibitory effect of AM compounds.	bind
49652	1	11183	7	10	NULL	NULL	NULL	leukemia cell line	Cell	murine	resistant to					E7010	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_jpn-j-cancer-res_92_7_11473728_s_6	11473728	A murine leukemia  cell line resistant to a sulfonamide antimitotic agent, E7010, which binds  to colchicine-binding sites on tubulin, was cross-resistant to the in  vitro growth-inhibitory effect of AM compounds.	bind
49653	2	11183	7	10	NULL	NULL	NULL	statement 1	Process		bind					tubulin	GP		colchicine-binding site		NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_jpn-j-cancer-res_92_7_11473728_s_6	11473728	A murine leukemia  cell line resistant to a sulfonamide antimitotic agent, E7010, which binds  to colchicine-binding sites on tubulin, was cross-resistant to the in  vitro growth-inhibitory effect of AM compounds.	bind
49654	3	11183	7	10	NULL	NULL	NULL	E7010	Chemical		is a type of					sulfonamide antimitotic agent	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_jpn-j-cancer-res_92_7_11473728_s_6	11473728	A murine leukemia  cell line resistant to a sulfonamide antimitotic agent, E7010, which binds  to colchicine-binding sites on tubulin, was cross-resistant to the in  vitro growth-inhibitory effect of AM compounds.	bind
49655	5	11183	7	10	NULL	NULL	NULL	statement 1	Process		cross-resistant to					statement 4	Process				NULL	in vitro	NULL	NULL	NULL	NULL	abs-batch0650-0679_jpn-j-cancer-res_92_7_11473728_s_6	11473728	A murine leukemia  cell line resistant to a sulfonamide antimitotic agent, E7010, which binds  to colchicine-binding sites on tubulin, was cross-resistant to the in  vitro growth-inhibitory effect of AM compounds.	bind
51528	4	11183	7	10	NULL	NULL	NULL	AM compounds	Chemical		inhibit					growth	Process				NULL	in vitro	NULL	NULL	NULL	NULL	abs-batch0650-0679_jpn-j-cancer-res_92_7_11473728_s_6	11473728	A murine leukemia  cell line resistant to a sulfonamide antimitotic agent, E7010, which binds  to colchicine-binding sites on tubulin, was cross-resistant to the in  vitro growth-inhibitory effect of AM compounds.	bind
43931	1	11184	6	10	NULL	NULL	NULL	laminin	GP		is a type of					non-collagenous protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_clinmicrobiolrev_13_3_470_s_4258	10885988	A murine nephritogenic monoclonal anti-DNA autoantibody binds directly to mouse laminin, the major non-collagenous protein component of the glomerular basement membrane.	bind
43941	2	11184	6	10	NULL	NULL	NULL	monoclonal anti-DNA autoantibody	GP	murine;; nephritogenic	bind		directly			laminin	GP	mouse			NULL		NULL	NULL	NULL	NULL	gw60_clinmicrobiolrev_13_3_470_s_4258	10885988	A murine nephritogenic monoclonal anti-DNA autoantibody binds directly to mouse laminin, the major non-collagenous protein component of the glomerular basement membrane.	bind
51529	3	11184	6	10	NULL	NULL	NULL	laminin	GP		is a component of					glomerular basement membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_clinmicrobiolrev_13_3_470_s_4258	10885988	A murine nephritogenic monoclonal anti-DNA autoantibody binds directly to mouse laminin, the major non-collagenous protein component of the glomerular basement membrane.	bind
49656	1	11184	7	10	NULL	NULL	NULL	monoclonal anti-DNA autoantibody 	GP	murine;;nephritogenic	bind		directly			laminin	GP	mouse			NULL		NULL	NULL	NULL	NULL	gw60_clinmicrobiolrev_13_3_470_s_4258	10885988	A murine nephritogenic monoclonal anti-DNA autoantibody binds directly to mouse laminin, the major non-collagenous protein component of the glomerular basement membrane.	bind
49657	2	11184	7	10	NULL	NULL	NULL	laminin	GP	mouse	is a type of					 non-collagenous protein 	GP				NULL		NULL	NULL	NULL	NULL	gw60_clinmicrobiolrev_13_3_470_s_4258	10885988	A murine nephritogenic monoclonal anti-DNA autoantibody binds directly to mouse laminin, the major non-collagenous protein component of the glomerular basement membrane.	bind
49658	3	11184	7	10	NULL	NULL	NULL	laminin	GP	mouse	is a component of					glomerular basement membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_clinmicrobiolrev_13_3_470_s_4258	10885988	A murine nephritogenic monoclonal anti-DNA autoantibody binds directly to mouse laminin, the major non-collagenous protein component of the glomerular basement membrane.	bind
44297	1	11185	6	10	NULL	NULL	NULL	actinin	GP		bind		may	C-terminal part of CH1 domain		actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_structure_6_11_1419_s_209	9817844	A mutagenesis study has identified residues within the C-terminal part of the   -actinin CH1 domain that may be involved in actin binding, as their substitution with alanine abolishes the interaction  [20]  .	bind
51530	2	11185	6	10	NULL	NULL	NULL	actinin	GP		is substituted with			C-terminal part of CH1 domain		alanine	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_structure_6_11_1419_s_209	9817844	A mutagenesis study has identified residues within the C-terminal part of the   -actinin CH1 domain that may be involved in actin binding, as their substitution with alanine abolishes the interaction  [20]  .	bind
51531	3	11185	6	10	NULL	NULL	NULL	statement 2	Process		abolishes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_structure_6_11_1419_s_209	9817844	A mutagenesis study has identified residues within the C-terminal part of the   -actinin CH1 domain that may be involved in actin binding, as their substitution with alanine abolishes the interaction  [20]  .	bind
49659	1	11185	7	10	NULL	NULL	NULL	actinin	GP		bind		may	C-terminal part of CH1 domain		actin	GP				NULL		NULL	NULL	NULL	NULL	gw60_structure_6_11_1419_s_209	9817844	A mutagenesis study has identified residues within the C-terminal part of the   -actinin CH1 domain that may be involved in actin binding, as their substitution with alanine abolishes the interaction  [20]  .	bind
49660	3	11185	7	10	NULL	NULL	NULL	statement 2	Process		abolishes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_structure_6_11_1419_s_209	9817844	A mutagenesis study has identified residues within the C-terminal part of the   -actinin CH1 domain that may be involved in actin binding, as their substitution with alanine abolishes the interaction  [20]  .	bind
49661	2	11185	7	10	NULL	NULL	NULL	actinin	GP		is substituted with			C-terminal part of CH1 domain 		alanine	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_structure_6_11_1419_s_209	9817844	A mutagenesis study has identified residues within the C-terminal part of the   -actinin CH1 domain that may be involved in actin binding, as their substitution with alanine abolishes the interaction  [20]  .	bind
43942	1	11186	6	10	NULL	NULL	NULL	E5 protein	GP	human papillomavirus type 16	bind					H+-ATPase	GP	vacuolar			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_virology_272_2_10873774_s_1	10873774	A mutagenic analysis of the E5 protein of human papillomavirus type 16 reveals that E5 binding to the vacuolar H+-ATPase is not sufficient for biological activity, using mammalian and yeast expression systems..	bind
43943	2	11186	6	10	NULL	NULL	NULL	statement 1	Process		is not sufficient for					biological activity	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_virology_272_2_10873774_s_1	10873774	A mutagenic analysis of the E5 protein of human papillomavirus type 16 reveals that E5 binding to the vacuolar H+-ATPase is not sufficient for biological activity, using mammalian and yeast expression systems..	bind
49672	1	11186	7	10	NULL	NULL	NULL	E5 protein	GP	human papillomavirus type 16	bind					H+-ATPase	GP	vacuolar			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_virology_272_2_10873774_s_1	10873774	A mutagenic analysis of the E5 protein of human papillomavirus type 16 reveals that E5 binding to the vacuolar H+-ATPase is not sufficient for biological activity, using mammalian and yeast expression systems..	bind
49673	2	11186	7	10	NULL	NULL	NULL	statement 1	Process		is not sufficient for					biological activity	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_virology_272_2_10873774_s_1	10873774	A mutagenic analysis of the E5 protein of human papillomavirus type 16 reveals that E5 binding to the vacuolar H+-ATPase is not sufficient for biological activity, using mammalian and yeast expression systems..	bind
44299	2	11187	6	10	NULL	NULL	NULL	statement 1	Process		is due to							disruption of		ISRE-like element	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_14_9344_s_192	9083071	A mutant  194 to  244 bp sequence unable to bind the BID2 complex due to disruption of the ISRE-like element ( 19) also was unable to compete for TF1phox binding.	bind
44300	1	11187	6	10	NULL	NULL	NULL			mutant	does not bind				194 to 244 bp sequence	BID2 complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_14_9344_s_192	9083071	A mutant  194 to  244 bp sequence unable to bind the BID2 complex due to disruption of the ISRE-like element ( 19) also was unable to compete for TF1phox binding.	bind
44301	3	11187	6	10	NULL	NULL	NULL	statement 1	Process		does not compete					TF1phox	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_14_9344_s_192	9083071	A mutant  194 to  244 bp sequence unable to bind the BID2 complex due to disruption of the ISRE-like element ( 19) also was unable to compete for TF1phox binding.	bind
49674	1	11187	7	10	NULL	NULL	NULL			mutant	does not bind				194 to 244 bp sequence	BID2 complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_14_9344_s_192	9083071	A mutant  194 to  244 bp sequence unable to bind the BID2 complex due to disruption of the ISRE-like element ( 19) also was unable to compete for TF1phox binding.	bind
49675	2	11187	7	10	NULL	NULL	NULL	statement 1	Process		due to							disruption of		ISRE-like element	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_14_9344_s_192	9083071	A mutant  194 to  244 bp sequence unable to bind the BID2 complex due to disruption of the ISRE-like element ( 19) also was unable to compete for TF1phox binding.	bind
49676	3	11187	7	10	NULL	NULL	NULL	statement 1	Process		does not compete with					TF1phox	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_14_9344_s_192	9083071	A mutant  194 to  244 bp sequence unable to bind the BID2 complex due to disruption of the ISRE-like element ( 19) also was unable to compete for TF1phox binding.	bind
43944	1	11188	6	10	NULL	NULL	NULL	B DNA	NucleicAcid	mutant	does not bind					myotrophin	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1589_3_247_s_274	12031792	A mutant  B DNA also did not show any binding to myotrophin.	bind
49677	1	11188	7	10	NULL	NULL	NULL	B DNA 	NucleicAcid	mutant	does not bind					myotrophin	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1589_3_247_s_274	12031792	A mutant  B DNA also did not show any binding to myotrophin.	bind
43945	1	11189	6	10	NULL	NULL	NULL	Mnk1	GP		bind					eIF4G	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_13_3465_s_9	10880459	A mutant adenovirus with a temperature-sensitive 100k protein that cannot inhibit cellular protein synthesis at restrictive temperature no longer blocks Mnk1 binding to eIF4G, or phosphorylation of eIF4E.	bind
43946	2	11189	6	10	NULL	NULL	NULL	100k protein	GP	mutant;; adenovirus	does not block					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_13_3465_s_9	10880459	A mutant adenovirus with a temperature-sensitive 100k protein that cannot inhibit cellular protein synthesis at restrictive temperature no longer blocks Mnk1 binding to eIF4G, or phosphorylation of eIF4E.	bind
43947	3	11189	6	10	NULL	NULL	NULL	100k protein	GP	mutant;; adenovirus	does not block					eIF4E	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_13_3465_s_9	10880459	A mutant adenovirus with a temperature-sensitive 100k protein that cannot inhibit cellular protein synthesis at restrictive temperature no longer blocks Mnk1 binding to eIF4G, or phosphorylation of eIF4E.	bind
43948	4	11189	6	10	NULL	NULL	NULL	100k protein	GP	mutant;; adenovirus	is sensitive to					temperature					NULL		NULL	NULL	NULL	NULL	gw60_embo_19_13_3465_s_9	10880459	A mutant adenovirus with a temperature-sensitive 100k protein that cannot inhibit cellular protein synthesis at restrictive temperature no longer blocks Mnk1 binding to eIF4G, or phosphorylation of eIF4E.	bind
43949	5	11189	6	10	NULL	NULL	NULL	100k protein	GP	mutant;; adenovirus	does not inhibit					cellular proteins	GP	synthesis of			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_13_3465_s_9	10880459	A mutant adenovirus with a temperature-sensitive 100k protein that cannot inhibit cellular protein synthesis at restrictive temperature no longer blocks Mnk1 binding to eIF4G, or phosphorylation of eIF4E.	bind
49678	1	11189	7	10	NULL	NULL	NULL	Mnk1	GP		bind					eIF4G	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_13_3465_s_9	10880459	A mutant adenovirus with a temperature-sensitive 100k protein that cannot inhibit cellular protein synthesis at restrictive temperature no longer blocks Mnk1 binding to eIF4G, or phosphorylation of eIF4E.	bind
49679	2	11189	7	10	NULL	NULL	NULL	100k protein	GP	mutant;;adenovirus	does not inhibit					cellular proteins	GP	synthesis of			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_13_3465_s_9	10880459	A mutant adenovirus with a temperature-sensitive 100k protein that cannot inhibit cellular protein synthesis at restrictive temperature no longer blocks Mnk1 binding to eIF4G, or phosphorylation of eIF4E.	bind
49680	3	11189	7	10	NULL	NULL	NULL	100k protein	GP	mutant;;adenovirus	does not block					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_13_3465_s_9	10880459	A mutant adenovirus with a temperature-sensitive 100k protein that cannot inhibit cellular protein synthesis at restrictive temperature no longer blocks Mnk1 binding to eIF4G, or phosphorylation of eIF4E.	bind
49681	4	11189	7	10	NULL	NULL	NULL	100k protein	GP	mutant;;adenovirus	does not block					eIF4E	GP	phosphorylation of 			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_13_3465_s_9	10880459	A mutant adenovirus with a temperature-sensitive 100k protein that cannot inhibit cellular protein synthesis at restrictive temperature no longer blocks Mnk1 binding to eIF4G, or phosphorylation of eIF4E.	bind
51532	5	11189	7	10	NULL	NULL	NULL	100k protein	GP	mutant;;adenovirus	is sensitive to					temperature					NULL		NULL	NULL	NULL	NULL	gw60_embo_19_13_3465_s_9	10880459	A mutant adenovirus with a temperature-sensitive 100k protein that cannot inhibit cellular protein synthesis at restrictive temperature no longer blocks Mnk1 binding to eIF4G, or phosphorylation of eIF4E.	bind
44302	1	11190	6	10	NULL	NULL	NULL	alpha-TM DY competitor	NucleicAcid	mutant	does not bind					PTB	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_2699_s_256	10082536	A mutant alpha-TM DY competitor which does not bind PTB, DYdeltaPC ( 20), was virtually ineffective in activating splicing (Fig.  6, lanes 11 and 12), as was an alpha-actinin competitor RNA truncated at the  ClaI site in the spacer and which therefore lacks UCUU motifs (lanes 13 and 14).	bind
44303	2	11190	6	10	NULL	NULL	NULL	alpha-TM DY competitor	NucleicAcid	mutant	does not bind					DYdeltaPC	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_2699_s_256	10082536	A mutant alpha-TM DY competitor which does not bind PTB, DYdeltaPC ( 20), was virtually ineffective in activating splicing (Fig.  6, lanes 11 and 12), as was an alpha-actinin competitor RNA truncated at the  ClaI site in the spacer and which therefore lacks UCUU motifs (lanes 13 and 14).	bind
44304	3	11190	6	10	NULL	NULL	NULL	alpha-TM DY competitor	NucleicAcid	mutant	does not activate					splicing	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_2699_s_256	10082536	A mutant alpha-TM DY competitor which does not bind PTB, DYdeltaPC ( 20), was virtually ineffective in activating splicing (Fig.  6, lanes 11 and 12), as was an alpha-actinin competitor RNA truncated at the  ClaI site in the spacer and which therefore lacks UCUU motifs (lanes 13 and 14).	bind
44305	4	11190	6	10	NULL	NULL	NULL	alpha-actinin competitor RNA	NucleicAcid		is truncated at									ClaI site in the spacer 	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_2699_s_256	10082536	A mutant alpha-TM DY competitor which does not bind PTB, DYdeltaPC ( 20), was virtually ineffective in activating splicing (Fig.  6, lanes 11 and 12), as was an alpha-actinin competitor RNA truncated at the  ClaI site in the spacer and which therefore lacks UCUU motifs (lanes 13 and 14).	bind
44306	5	11190	6	10	NULL	NULL	NULL	statement 4	Process		lacks									UCUU motifs	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_2699_s_256	10082536	A mutant alpha-TM DY competitor which does not bind PTB, DYdeltaPC ( 20), was virtually ineffective in activating splicing (Fig.  6, lanes 11 and 12), as was an alpha-actinin competitor RNA truncated at the  ClaI site in the spacer and which therefore lacks UCUU motifs (lanes 13 and 14).	bind
51533	6	11190	6	10	NULL	NULL	NULL	alpha-TM DY competitor	NucleicAcid	mutant	is a type of					statement 4	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_2699_s_256	10082536	A mutant alpha-TM DY competitor which does not bind PTB, DYdeltaPC ( 20), was virtually ineffective in activating splicing (Fig.  6, lanes 11 and 12), as was an alpha-actinin competitor RNA truncated at the  ClaI site in the spacer and which therefore lacks UCUU motifs (lanes 13 and 14).	bind
49682	1	11190	7	10	NULL	NULL	NULL	alpha-TM DY competitor	NucleicAcid	mutant	does not bind					PTB	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_2699_s_256	10082536	A mutant alpha-TM DY competitor which does not bind PTB, DYdeltaPC ( 20), was virtually ineffective in activating splicing (Fig.  6, lanes 11 and 12), as was an alpha-actinin competitor RNA truncated at the  ClaI site in the spacer and which therefore lacks UCUU motifs (lanes 13 and 14).	bind
49683	2	11190	7	10	NULL	NULL	NULL	alpha-TM DY competitor	NucleicAcid	mutant	does not bind					DYdeltaPC	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_2699_s_256	10082536	A mutant alpha-TM DY competitor which does not bind PTB, DYdeltaPC ( 20), was virtually ineffective in activating splicing (Fig.  6, lanes 11 and 12), as was an alpha-actinin competitor RNA truncated at the  ClaI site in the spacer and which therefore lacks UCUU motifs (lanes 13 and 14).	bind
49684	3	11190	7	10	NULL	NULL	NULL	alpha-TM DY alpha-TM DY competitor	NucleicAcid	mutant	does not activate					splicing	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_2699_s_256	10082536	A mutant alpha-TM DY competitor which does not bind PTB, DYdeltaPC ( 20), was virtually ineffective in activating splicing (Fig.  6, lanes 11 and 12), as was an alpha-actinin competitor RNA truncated at the  ClaI site in the spacer and which therefore lacks UCUU motifs (lanes 13 and 14).	bind
51534	4	11190	7	10	NULL	NULL	NULL	alpha-actinin competitor RNA	NucleicAcid		is truncated at									ClaI site in the spacer	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_2699_s_256	10082536	A mutant alpha-TM DY competitor which does not bind PTB, DYdeltaPC ( 20), was virtually ineffective in activating splicing (Fig.  6, lanes 11 and 12), as was an alpha-actinin competitor RNA truncated at the  ClaI site in the spacer and which therefore lacks UCUU motifs (lanes 13 and 14).	bind
51535	5	11190	7	10	NULL	NULL	NULL	statement 4	Process		lacks									UCUU motifs	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_2699_s_256	10082536	A mutant alpha-TM DY competitor which does not bind PTB, DYdeltaPC ( 20), was virtually ineffective in activating splicing (Fig.  6, lanes 11 and 12), as was an alpha-actinin competitor RNA truncated at the  ClaI site in the spacer and which therefore lacks UCUU motifs (lanes 13 and 14).	bind
51536	6	11190	7	10	NULL	NULL	NULL	alpha-TM DY competitor	NucleicAcid	mutant	is a type of					statement 4	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_2699_s_256	10082536	A mutant alpha-TM DY competitor which does not bind PTB, DYdeltaPC ( 20), was virtually ineffective in activating splicing (Fig.  6, lanes 11 and 12), as was an alpha-actinin competitor RNA truncated at the  ClaI site in the spacer and which therefore lacks UCUU motifs (lanes 13 and 14).	bind
43950	2	11191	6	10	NULL	NULL	NULL	statement 1	Process		bind		noncovalently			apo(a)	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_502_s_19	12615683	A mutant apoB lacking Cys4326 still binds apo(a) noncovalently despite being unable to form the disulphide bond.	bind
43951	3	11191	6	10	NULL	NULL	NULL	statement 1	Process		does not form					disulphide bond					NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_502_s_19	12615683	A mutant apoB lacking Cys4326 still binds apo(a) noncovalently despite being unable to form the disulphide bond.	bind
51537	1	11191	6	10	NULL	NULL	NULL	apoB	GP	mutant	lacks					Cys4326	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_502_s_19	12615683	A mutant apoB lacking Cys4326 still binds apo(a) noncovalently despite being unable to form the disulphide bond.	bind
49685	1	11191	7	10	NULL	NULL	NULL	apoB	GP	mutant	lacks					Cys4326 	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_502_s_19	12615683	A mutant apoB lacking Cys4326 still binds apo(a) noncovalently despite being unable to form the disulphide bond.	bind
49686	2	11191	7	10	NULL	NULL	NULL	statement 1	Process		bind		noncovalently			apo(a) 	GP				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_502_s_19	12615683	A mutant apoB lacking Cys4326 still binds apo(a) noncovalently despite being unable to form the disulphide bond.	bind
49687	3	11191	7	10	NULL	NULL	NULL	statement 1	Process		does not form					disulphide bond					NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_23_3_502_s_19	12615683	A mutant apoB lacking Cys4326 still binds apo(a) noncovalently despite being unable to form the disulphide bond.	bind
43952	1	11192	6	10	NULL	NULL	NULL	 BAK peptide	AminoAcid	mutant	bind		decreased	R76A		BCL-XL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_39_24101_s_91	9305851	A mutant BAK R76A peptide demonstrated decreased binding to BCL-XL ( 17).	bind
49688	1	11192	7	10	NULL	NULL	NULL	BAK peptide	AminoAcid	mutant	bind		decreased	R76A		BCL-XL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_39_24101_s_91	9305851	A mutant BAK R76A peptide demonstrated decreased binding to BCL-XL ( 17).	bind
44988	1	11193	6	10	NULL	NULL	NULL	G-kinase	GP		regulates					c-Raf	GP		Ser43		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6983_s_7	9819386	A mutant c-Raf kinase with an Ala substitution for Ser43 was insensitive to inhibition by cGMP and G-kinase, and expression of this mutant kinase protected cells from inhibition of EGF-induced MAP kinase activity by cGMP and G-kinase, suggesting that Ser43 in c-Raf is the major target for regulation by G-kinase.	bind
44989	2	11193	6	10	NULL	NULL	NULL	EGF	GP		induces					MAP kinase 	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6983_s_7	9819386	A mutant c-Raf kinase with an Ala substitution for Ser43 was insensitive to inhibition by cGMP and G-kinase, and expression of this mutant kinase protected cells from inhibition of EGF-induced MAP kinase activity by cGMP and G-kinase, suggesting that Ser43 in c-Raf is the major target for regulation by G-kinase.	bind
44990	3	11193	6	10	NULL	NULL	NULL	cGMP	Chemical		inhibits					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6983_s_7	9819386	A mutant c-Raf kinase with an Ala substitution for Ser43 was insensitive to inhibition by cGMP and G-kinase, and expression of this mutant kinase protected cells from inhibition of EGF-induced MAP kinase activity by cGMP and G-kinase, suggesting that Ser43 in c-Raf is the major target for regulation by G-kinase.	bind
44991	4	11193	6	10	NULL	NULL	NULL	G-kinase	GP		inhibits					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6983_s_7	9819386	A mutant c-Raf kinase with an Ala substitution for Ser43 was insensitive to inhibition by cGMP and G-kinase, and expression of this mutant kinase protected cells from inhibition of EGF-induced MAP kinase activity by cGMP and G-kinase, suggesting that Ser43 in c-Raf is the major target for regulation by G-kinase.	bind
44992	5	11193	6	10	NULL	NULL	NULL	c-Raf	GP		is a type of					kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6983_s_7	9819386	A mutant c-Raf kinase with an Ala substitution for Ser43 was insensitive to inhibition by cGMP and G-kinase, and expression of this mutant kinase protected cells from inhibition of EGF-induced MAP kinase activity by cGMP and G-kinase, suggesting that Ser43 in c-Raf is the major target for regulation by G-kinase.	bind
44993	6	11193	6	10	NULL	NULL	NULL	c-Raf	GP		is substituted by			Ser43		c-Raf	GP		Ala		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6983_s_7	9819386	A mutant c-Raf kinase with an Ala substitution for Ser43 was insensitive to inhibition by cGMP and G-kinase, and expression of this mutant kinase protected cells from inhibition of EGF-induced MAP kinase activity by cGMP and G-kinase, suggesting that Ser43 in c-Raf is the major target for regulation by G-kinase.	bind
44995	7	11193	6	10	NULL	NULL	NULL	statement 6	Process		protects					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6983_s_7	9819386	A mutant c-Raf kinase with an Ala substitution for Ser43 was insensitive to inhibition by cGMP and G-kinase, and expression of this mutant kinase protected cells from inhibition of EGF-induced MAP kinase activity by cGMP and G-kinase, suggesting that Ser43 in c-Raf is the major target for regulation by G-kinase.	bind
44996	8	11193	6	10	NULL	NULL	NULL	statement 6	Process		protects					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6983_s_7	9819386	A mutant c-Raf kinase with an Ala substitution for Ser43 was insensitive to inhibition by cGMP and G-kinase, and expression of this mutant kinase protected cells from inhibition of EGF-induced MAP kinase activity by cGMP and G-kinase, suggesting that Ser43 in c-Raf is the major target for regulation by G-kinase.	bind
49738	1	11193	7	10	NULL	NULL	NULL	c-Raf kinase	GP		is substituted with			Ser43		c-Raf kinase	GP		Ala		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6983_s_7	9819386	A mutant c-Raf kinase with an Ala substitution for Ser43 was insensitive to inhibition by cGMP and G-kinase, and expression of this mutant kinase protected cells from inhibition of EGF-induced MAP kinase activity by cGMP and G-kinase, suggesting that Ser43 in c-Raf is the major target for regulation by G-kinase.	bind
49740	2	11193	7	10	NULL	NULL	NULL	EGF	GP		induce					MAP kinase	GP	activity of 			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6983_s_7	9819386	A mutant c-Raf kinase with an Ala substitution for Ser43 was insensitive to inhibition by cGMP and G-kinase, and expression of this mutant kinase protected cells from inhibition of EGF-induced MAP kinase activity by cGMP and G-kinase, suggesting that Ser43 in c-Raf is the major target for regulation by G-kinase.	bind
49741	3	11193	7	10	NULL	NULL	NULL	cGMP	Chemical		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6983_s_7	9819386	A mutant c-Raf kinase with an Ala substitution for Ser43 was insensitive to inhibition by cGMP and G-kinase, and expression of this mutant kinase protected cells from inhibition of EGF-induced MAP kinase activity by cGMP and G-kinase, suggesting that Ser43 in c-Raf is the major target for regulation by G-kinase.	bind
49742	4	11193	7	10	NULL	NULL	NULL	G-kinase	GP		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6983_s_7	9819386	A mutant c-Raf kinase with an Ala substitution for Ser43 was insensitive to inhibition by cGMP and G-kinase, and expression of this mutant kinase protected cells from inhibition of EGF-induced MAP kinase activity by cGMP and G-kinase, suggesting that Ser43 in c-Raf is the major target for regulation by G-kinase.	bind
49743	7	11193	7	10	NULL	NULL	NULL	G-kinase	GP		regulates					C-Raf	GP		Ser43		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6983_s_7	9819386	A mutant c-Raf kinase with an Ala substitution for Ser43 was insensitive to inhibition by cGMP and G-kinase, and expression of this mutant kinase protected cells from inhibition of EGF-induced MAP kinase activity by cGMP and G-kinase, suggesting that Ser43 in c-Raf is the major target for regulation by G-kinase.	bind
51756	5	11193	7	10	NULL	NULL	NULL	statement 1	Process		protect					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6983_s_7	9819386	A mutant c-Raf kinase with an Ala substitution for Ser43 was insensitive to inhibition by cGMP and G-kinase, and expression of this mutant kinase protected cells from inhibition of EGF-induced MAP kinase activity by cGMP and G-kinase, suggesting that Ser43 in c-Raf is the major target for regulation by G-kinase.	bind
51758	6	11193	7	10	NULL	NULL	NULL	statement 1	Process		protect					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6983_s_7	9819386	A mutant c-Raf kinase with an Ala substitution for Ser43 was insensitive to inhibition by cGMP and G-kinase, and expression of this mutant kinase protected cells from inhibition of EGF-induced MAP kinase activity by cGMP and G-kinase, suggesting that Ser43 in c-Raf is the major target for regulation by G-kinase.	bind
43955	1	11194	6	NULL	NULL	0	NULL		NULL		is changed to	NULL		Arg66			NULL		Glu		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_27_19237_s_285	10383431	A mutant carrying the combined change of Arg66 to Glu and His67 to Thr demonstrated decreased binding to C4b-Sepharose at physiological ionic strength.	bind
43956	2	11194	6	NULL	NULL	0	NULL		NULL		is changed to	NULL		His67			NULL		Thr		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_27_19237_s_285	10383431	A mutant carrying the combined change of Arg66 to Glu and His67 to Thr demonstrated decreased binding to C4b-Sepharose at physiological ionic strength.	bind
43957	3	11194	6	10	NULL	NULL	NULL	statement 1	Process		occurs in concert with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_27_19237_s_285	10383431	A mutant carrying the combined change of Arg66 to Glu and His67 to Thr demonstrated decreased binding to C4b-Sepharose at physiological ionic strength.	bind
43958	4	11194	6	10	NULL	NULL	NULL	statement 3	Process		bind		less avidly			C4b	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_27_19237_s_285	10383431	A mutant carrying the combined change of Arg66 to Glu and His67 to Thr demonstrated decreased binding to C4b-Sepharose at physiological ionic strength.	bind
51543	1	11194	7	10	NULL	0	NULL		NULL		is changed to	NULL		Arg66 			NULL		Glu 		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_27_19237_s_285	10383431	A mutant carrying the combined change of Arg66 to Glu and His67 to Thr demonstrated decreased binding to C4b-Sepharose at physiological ionic strength.	bind
51544	2	11194	7	10	NULL	0	NULL		NULL		is changed to	NULL		His67			NULL		Thr		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_27_19237_s_285	10383431	A mutant carrying the combined change of Arg66 to Glu and His67 to Thr demonstrated decreased binding to C4b-Sepharose at physiological ionic strength.	bind
51545	3	11194	7	10	NULL	NULL	NULL	statement 1	Process		occurs in concert with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_27_19237_s_285	10383431	A mutant carrying the combined change of Arg66 to Glu and His67 to Thr demonstrated decreased binding to C4b-Sepharose at physiological ionic strength.	bind
51546	4	11194	7	10	NULL	NULL	NULL	statement 3	Process		bind		less avidly			C4b	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_27_19237_s_285	10383431	A mutant carrying the combined change of Arg66 to Glu and His67 to Thr demonstrated decreased binding to C4b-Sepharose at physiological ionic strength.	bind
43959	1	11195	6	10	NULL	NULL	NULL	CD-R1	GP		is mutated to			C-tail tyrosine		CD-R1	GP		phenylalanine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_11_7771_s_228	10713090	A mutant CD-R1 with both C-tail tyrosine residues mutated to phenylalanine failed to bind to Grb14, but the independent Y766F and Y776F receptor constructs bound to Grb14 with strength equal to the wild-type CD-R1.	bind
43960	2	11195	6	10	NULL	NULL	NULL	statement 1	Process		does not bind					Grb14	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_11_7771_s_228	10713090	A mutant CD-R1 with both C-tail tyrosine residues mutated to phenylalanine failed to bind to Grb14, but the independent Y766F and Y776F receptor constructs bound to Grb14 with strength equal to the wild-type CD-R1.	bind
43961	3	11195	6	10	NULL	NULL	NULL	CD-R1	GP	wild type	bind					Grb14	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_11_7771_s_228	10713090	A mutant CD-R1 with both C-tail tyrosine residues mutated to phenylalanine failed to bind to Grb14, but the independent Y766F and Y776F receptor constructs bound to Grb14 with strength equal to the wild-type CD-R1.	bind
43962	4	11195	6	10	NULL	NULL	NULL	receptor construct	AminoAcid		bind			Y766F		Grb14	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_11_7771_s_228	10713090	A mutant CD-R1 with both C-tail tyrosine residues mutated to phenylalanine failed to bind to Grb14, but the independent Y766F and Y776F receptor constructs bound to Grb14 with strength equal to the wild-type CD-R1.	bind
43963	5	11195	6	10	NULL	NULL	NULL	receptor construct	AminoAcid		bind			Y776F		Grb14	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_11_7771_s_228	10713090	A mutant CD-R1 with both C-tail tyrosine residues mutated to phenylalanine failed to bind to Grb14, but the independent Y766F and Y776F receptor constructs bound to Grb14 with strength equal to the wild-type CD-R1.	bind
43964	6	11195	6	10	NULL	NULL	NULL	statement 4	Process	affinity of	is equal to					statement 3	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_11_7771_s_228	10713090	A mutant CD-R1 with both C-tail tyrosine residues mutated to phenylalanine failed to bind to Grb14, but the independent Y766F and Y776F receptor constructs bound to Grb14 with strength equal to the wild-type CD-R1.	bind
43965	7	11195	6	10	NULL	NULL	NULL	statement 5	Process	affinity of	is equal to					statement 3	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_11_7771_s_228	10713090	A mutant CD-R1 with both C-tail tyrosine residues mutated to phenylalanine failed to bind to Grb14, but the independent Y766F and Y776F receptor constructs bound to Grb14 with strength equal to the wild-type CD-R1.	bind
49746	1	11195	7	10	NULL	NULL	NULL	statement 5	Process		does not bind					Grb14	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_11_7771_s_228	10713090	A mutant CD-R1 with both C-tail tyrosine residues mutated to phenylalanine failed to bind to Grb14, but the independent Y766F and Y776F receptor constructs bound to Grb14 with strength equal to the wild-type CD-R1.	bind
49747	2	11195	7	10	NULL	NULL	NULL	receptor construct	AminoAcid		bind			Y766F		Grb14	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_11_7771_s_228	10713090	A mutant CD-R1 with both C-tail tyrosine residues mutated to phenylalanine failed to bind to Grb14, but the independent Y766F and Y776F receptor constructs bound to Grb14 with strength equal to the wild-type CD-R1.	bind
49748	3	11195	7	10	NULL	NULL	NULL	receptor construct	AminoAcid		bind			Y776F		Grb14	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_11_7771_s_228	10713090	A mutant CD-R1 with both C-tail tyrosine residues mutated to phenylalanine failed to bind to Grb14, but the independent Y766F and Y776F receptor constructs bound to Grb14 with strength equal to the wild-type CD-R1.	bind
49749	4	11195	7	10	NULL	NULL	NULL	CD-R1 receptor	GP	wild-type	bind					Grb14	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_11_7771_s_228	10713090	A mutant CD-R1 with both C-tail tyrosine residues mutated to phenylalanine failed to bind to Grb14, but the independent Y766F and Y776F receptor constructs bound to Grb14 with strength equal to the wild-type CD-R1.	bind
51540	5	11195	7	10	NULL	NULL	NULL	CD-R1	GP		is mutated to			C-tail tyrosine		CD-R1	GP		phenylalanine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_11_7771_s_228	10713090	A mutant CD-R1 with both C-tail tyrosine residues mutated to phenylalanine failed to bind to Grb14, but the independent Y766F and Y776F receptor constructs bound to Grb14 with strength equal to the wild-type CD-R1.	bind
51541	6	11195	7	10	NULL	NULL	NULL	statement 2	Process	affinity of	is equivalent to					statement 4	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_11_7771_s_228	10713090	A mutant CD-R1 with both C-tail tyrosine residues mutated to phenylalanine failed to bind to Grb14, but the independent Y766F and Y776F receptor constructs bound to Grb14 with strength equal to the wild-type CD-R1.	bind
51542	7	11195	7	10	NULL	NULL	NULL	statement 3	Process	affinity of	is equivalent to					statement 4	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_11_7771_s_228	10713090	A mutant CD-R1 with both C-tail tyrosine residues mutated to phenylalanine failed to bind to Grb14, but the independent Y766F and Y776F receptor constructs bound to Grb14 with strength equal to the wild-type CD-R1.	bind
43966	1	11196	6	10	NULL	NULL	NULL	cholera toxin	GP	mutant	bind			 B subunit		GM1- ganglioside	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_4_905_s_623	9585410	A mutant cholera toxin B subunit that binds GM1- ganglioside but lacks immunomodulatory or toxic activity.	bind
43967	2	11196	6	10	NULL	NULL	NULL	statement 1	Process		lacks					immunomodulatory activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_4_905_s_623	9585410	A mutant cholera toxin B subunit that binds GM1- ganglioside but lacks immunomodulatory or toxic activity.	bind
43968	3	11196	6	10	NULL	NULL	NULL	statement 1	Process		lacks					toxic activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_4_905_s_623	9585410	A mutant cholera toxin B subunit that binds GM1- ganglioside but lacks immunomodulatory or toxic activity.	bind
49750	1	11196	7	10	NULL	NULL	NULL	cholera toxin	GP	mutant	bind			B subunit 		GM1- ganglioside	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_4_905_s_623	9585410	A mutant cholera toxin B subunit that binds GM1- ganglioside but lacks immunomodulatory or toxic activity.	bind
49751	2	11196	7	10	NULL	NULL	NULL	statement 1	Process		lacks					immunomodulatory activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_4_905_s_623	9585410	A mutant cholera toxin B subunit that binds GM1- ganglioside but lacks immunomodulatory or toxic activity.	bind
49752	3	11196	7	10	NULL	NULL	NULL	statement 1	Process		lacks					toxic activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_141_4_905_s_623	9585410	A mutant cholera toxin B subunit that binds GM1- ganglioside but lacks immunomodulatory or toxic activity.	bind
44330	1	11198	6	10	NULL	NULL	NULL	GATA-3	GP		bind									CIRE	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_31_28177_s_175	15941711	A mutant CIRE with 12 instead of 6 nucleotides separating the GATA-binding motifs can no longer inhibit binding of GATA-3 to the CIRE efficiently ( Fig. 5 B,  lane 3), and a mutant with an inverted 3' GATA-binding motif also cannot inhibit binding of CIRE to nuclear proteins of Th2 cells ( Fig. 5 B,  lane 4).	bind
44331	2	11198	6	10	NULL	NULL	NULL	nuclear proteins	GP		bind									CIRE	NULL	Th2 cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_31_28177_s_175	15941711	A mutant CIRE with 12 instead of 6 nucleotides separating the GATA-binding motifs can no longer inhibit binding of GATA-3 to the CIRE efficiently ( Fig. 5 B,  lane 3), and a mutant with an inverted 3' GATA-binding motif also cannot inhibit binding of CIRE to nuclear proteins of Th2 cells ( Fig. 5 B,  lane 4).	bind
44332	3	11198	6	10	NULL	NULL	NULL			mutant	does not inhibit		efficiently		CIRE	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_31_28177_s_175	15941711	A mutant CIRE with 12 instead of 6 nucleotides separating the GATA-binding motifs can no longer inhibit binding of GATA-3 to the CIRE efficiently ( Fig. 5 B,  lane 3), and a mutant with an inverted 3' GATA-binding motif also cannot inhibit binding of CIRE to nuclear proteins of Th2 cells ( Fig. 5 B,  lane 4).	bind
44333	4	11198	6	10	NULL	NULL	NULL			mutant	does not inhibit				inverted 3' GATA-binding motif 	statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_31_28177_s_175	15941711	A mutant CIRE with 12 instead of 6 nucleotides separating the GATA-binding motifs can no longer inhibit binding of GATA-3 to the CIRE efficiently ( Fig. 5 B,  lane 3), and a mutant with an inverted 3' GATA-binding motif also cannot inhibit binding of CIRE to nuclear proteins of Th2 cells ( Fig. 5 B,  lane 4).	bind
49753	1	11198	7	10	NULL	NULL	NULL	GATA-3	GP		bind									CIRE	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_31_28177_s_175	15941711	A mutant CIRE with 12 instead of 6 nucleotides separating the GATA-binding motifs can no longer inhibit binding of GATA-3 to the CIRE efficiently ( Fig. 5 B,  lane 3), and a mutant with an inverted 3' GATA-binding motif also cannot inhibit binding of CIRE to nuclear proteins of Th2 cells ( Fig. 5 B,  lane 4).	bind
49754	2	11198	7	10	NULL	NULL	NULL			mutant	does not inhibit		efficiently		CIRE	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_31_28177_s_175	15941711	A mutant CIRE with 12 instead of 6 nucleotides separating the GATA-binding motifs can no longer inhibit binding of GATA-3 to the CIRE efficiently ( Fig. 5 B,  lane 3), and a mutant with an inverted 3' GATA-binding motif also cannot inhibit binding of CIRE to nuclear proteins of Th2 cells ( Fig. 5 B,  lane 4).	bind
49755	3	11198	7	10	NULL	NULL	NULL				bind				CIRE	nuclear proteins	GP				NULL	Th2 cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_31_28177_s_175	15941711	A mutant CIRE with 12 instead of 6 nucleotides separating the GATA-binding motifs can no longer inhibit binding of GATA-3 to the CIRE efficiently ( Fig. 5 B,  lane 3), and a mutant with an inverted 3' GATA-binding motif also cannot inhibit binding of CIRE to nuclear proteins of Th2 cells ( Fig. 5 B,  lane 4).	bind
49756	4	11198	7	10	NULL	NULL	NULL			mutant	does not inhibit				inverted 3' GATA-binding motif	statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_31_28177_s_175	15941711	A mutant CIRE with 12 instead of 6 nucleotides separating the GATA-binding motifs can no longer inhibit binding of GATA-3 to the CIRE efficiently ( Fig. 5 B,  lane 3), and a mutant with an inverted 3' GATA-binding motif also cannot inhibit binding of CIRE to nuclear proteins of Th2 cells ( Fig. 5 B,  lane 4).	bind
43969	1	11199	6	10	NULL	NULL	NULL	DDB2	GP	mutant	does not bind					Cul-4A	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_20_6738_s_254	11564859	A mutant DDB2 (2RO) which does not bind Cul-4A did not exhibit any significant increase in ubiquitination by the coexpression of Cul-4A.	bind
43970	2	11199	6	10	NULL	NULL	NULL	DDB2	GP	mutant	is					2RO	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_20_6738_s_254	11564859	A mutant DDB2 (2RO) which does not bind Cul-4A did not exhibit any significant increase in ubiquitination by the coexpression of Cul-4A.	bind
43971	3	11199	6	10	NULL	NULL	NULL	DDB2	GP	mutant	is coexpressed with					Cul-4A	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_20_6738_s_254	11564859	A mutant DDB2 (2RO) which does not bind Cul-4A did not exhibit any significant increase in ubiquitination by the coexpression of Cul-4A.	bind
43972	4	11199	6	10	NULL	NULL	NULL	statement 3	Process		does not increase		significantly			ubiquitination	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_20_6738_s_254	11564859	A mutant DDB2 (2RO) which does not bind Cul-4A did not exhibit any significant increase in ubiquitination by the coexpression of Cul-4A.	bind
49757	1	11199	7	10	NULL	NULL	NULL	DDB2	GP	mutant	does not bind					Cul-4A	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_20_6738_s_254	11564859	A mutant DDB2 (2RO) which does not bind Cul-4A did not exhibit any significant increase in ubiquitination by the coexpression of Cul-4A.	bind
49758	2	11199	7	10	NULL	NULL	NULL	DDB2	GP	mutant	does not increase					ubiquitination	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_20_6738_s_254	11564859	A mutant DDB2 (2RO) which does not bind Cul-4A did not exhibit any significant increase in ubiquitination by the coexpression of Cul-4A.	bind
49759	3	11199	7	10	NULL	NULL	NULL	statement 2	Process		occur upon					Cul-4A	GP	coexpression of 			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_20_6738_s_254	11564859	A mutant DDB2 (2RO) which does not bind Cul-4A did not exhibit any significant increase in ubiquitination by the coexpression of Cul-4A.	bind
49760	4	11199	7	10	NULL	NULL	NULL	DDB2	GP	mutant	is					2RO	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_20_6738_s_254	11564859	A mutant DDB2 (2RO) which does not bind Cul-4A did not exhibit any significant increase in ubiquitination by the coexpression of Cul-4A.	bind
43973	1	11200	6	10	NULL	NULL	NULL	FnbA	GP	defective mutant	bind					Fn	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_6_2933_s_260	12010982	A mutant defective in both FnbA and FnbB ( 13) still shows residual binding to Fn ( 7), and it is possible that surface-associated Eap contributes to this binding.	bind
43974	2	11200	6	10	NULL	NULL	NULL	Eap	GP	surface associated	contributes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_6_2933_s_260	12010982	A mutant defective in both FnbA and FnbB ( 13) still shows residual binding to Fn ( 7), and it is possible that surface-associated Eap contributes to this binding.	bind
51538	3	11200	6	10	NULL	NULL	NULL	FnbB	GP	defective mutant	bind					Fn	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_6_2933_s_260	12010982	A mutant defective in both FnbA and FnbB ( 13) still shows residual binding to Fn ( 7), and it is possible that surface-associated Eap contributes to this binding.	bind
51539	4	11200	6	10	NULL	NULL	NULL	Eap	GP	surface associated	contribute to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_6_2933_s_260	12010982	A mutant defective in both FnbA and FnbB ( 13) still shows residual binding to Fn ( 7), and it is possible that surface-associated Eap contributes to this binding.	bind
49761	1	11200	7	10	NULL	NULL	NULL	FnbA	GP	defective mutant	bind					Fn	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_6_2933_s_260	12010982	A mutant defective in both FnbA and FnbB ( 13) still shows residual binding to Fn ( 7), and it is possible that surface-associated Eap contributes to this binding.	bind
49762	2	11200	7	10	NULL	NULL	NULL	FnbB	GP	defective mutant	bind					Fn	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_6_2933_s_260	12010982	A mutant defective in both FnbA and FnbB ( 13) still shows residual binding to Fn ( 7), and it is possible that surface-associated Eap contributes to this binding.	bind
49763	3	11200	7	10	NULL	NULL	NULL	Eap	GP	surface-associated	contribute to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_6_2933_s_260	12010982	A mutant defective in both FnbA and FnbB ( 13) still shows residual binding to Fn ( 7), and it is possible that surface-associated Eap contributes to this binding.	bind
49764	4	11200	7	10	NULL	NULL	NULL	Eap	GP	surface-associated	contribute to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_70_6_2933_s_260	12010982	A mutant defective in both FnbA and FnbB ( 13) still shows residual binding to Fn ( 7), and it is possible that surface-associated Eap contributes to this binding.	bind
44417	1	11201	5	10	NULL	NULL	NULL	Clock	GP	Drosophila	is a homolog of					Clock	GP	mammalian			NULL		NULL	NULL	NULL	NULL	gw60_cell_103_7_1009_s_232	11163178	A mutant Drosophila homolog of mammalian  Clock disrupts circadian rhythms and transcription of  period and  timeless.	bind
44418	2	11201	5	10	NULL	NULL	NULL	statement 1	Process	mutant	disrupt					circadian rhythms	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_7_1009_s_232	11163178	A mutant Drosophila homolog of mammalian  Clock disrupts circadian rhythms and transcription of  period and  timeless.	bind
44419	3	11201	5	10	NULL	NULL	NULL	statement 1	Process	mutant	disrupt					period	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw60_cell_103_7_1009_s_232	11163178	A mutant Drosophila homolog of mammalian  Clock disrupts circadian rhythms and transcription of  period and  timeless.	bind
44420	4	11201	5	10	NULL	NULL	NULL	statement 1	Process	mutant	disrupt					timeless	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw60_cell_103_7_1009_s_232	11163178	A mutant Drosophila homolog of mammalian  Clock disrupts circadian rhythms and transcription of  period and  timeless.	bind
44334	1	11201	6	10	NULL	NULL	NULL	Clock	GP	Drosophila 	is a homolog of					Clock	GP	mammalian			NULL		NULL	NULL	NULL	NULL	gw60_cell_103_7_1009_s_232	11163178	A mutant Drosophila homolog of mammalian  Clock disrupts circadian rhythms and transcription of  period and  timeless.	bind
44335	2	11201	6	10	NULL	NULL	NULL	statement 1	Process	mutant	disrupts					circadian rhythms	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_7_1009_s_232	11163178	A mutant Drosophila homolog of mammalian  Clock disrupts circadian rhythms and transcription of  period and  timeless.	bind
44336	3	11201	6	10	NULL	NULL	NULL	Clock	GP	mutant	disrupts					period	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw60_cell_103_7_1009_s_232	11163178	A mutant Drosophila homolog of mammalian  Clock disrupts circadian rhythms and transcription of  period and  timeless.	bind
50850	4	11201	6	10	NULL	NULL	NULL	statement 1	Process	mutant	disrupts					timeless	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw60_cell_103_7_1009_s_232	11163178	A mutant Drosophila homolog of mammalian  Clock disrupts circadian rhythms and transcription of  period and  timeless.	bind
44421	1	11202	5	10	NULL	NULL	NULL	E1A	GP	mutant	does not bind				exon 2	CtBP	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10379_s_297	16287852	A mutant E1A exon 2 that no longerR binds to CtBP, however, had no effect on transcriptional activity of the  Hey1 promoter.	bind
44422	2	11202	5	10	NULL	NULL	NULL	E1A	GP	mutant	does not effect				exon 2	Hey1	GP	transcriptional activity of		promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10379_s_297	16287852	A mutant E1A exon 2 that no longerR binds to CtBP, however, had no effect on transcriptional activity of the  Hey1 promoter.	bind
44337	1	11202	6	10	NULL	NULL	NULL	E1A 	GP	mutant	does not bind				exon 2	CtBP	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10379_s_297	16287852	A mutant E1A exon 2 that no longerR binds to CtBP, however, had no effect on transcriptional activity of the  Hey1 promoter.	bind
44338	2	11202	6	10	NULL	NULL	NULL	E1A 	GP	mutant	has no effect on				exon 2	Hey1	GP	transcriptional activity of		promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_23_10379_s_297	16287852	A mutant E1A exon 2 that no longerR binds to CtBP, however, had no effect on transcriptional activity of the  Hey1 promoter.	bind
44423	1	11204	5	10	NULL	NULL	NULL	ABCA1	GP	mutant	bind			W590S		apoA-I	GP				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_45_2_287_s_8	14617740	A mutant form of ABCA1 (W590S) that avidly binds apoA-I but fails to promote cholesterol efflux released apoA-I with similar kinetics but without transfer of cholesterol to apoA-I.	bind
44424	2	11204	5	10	NULL	NULL	NULL	ABCA1	GP	mutant	does not promote			W590S		cholesterol efflux	Process				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_45_2_287_s_8	14617740	A mutant form of ABCA1 (W590S) that avidly binds apoA-I but fails to promote cholesterol efflux released apoA-I with similar kinetics but without transfer of cholesterol to apoA-I.	bind
44425	3	11204	5	10	NULL	NULL	NULL	ABCA1	GP	mutant	release			W590S		apoA-I	GP				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_45_2_287_s_8	14617740	A mutant form of ABCA1 (W590S) that avidly binds apoA-I but fails to promote cholesterol efflux released apoA-I with similar kinetics but without transfer of cholesterol to apoA-I.	bind
44426	4	11204	5	10	NULL	NULL	NULL	cholesterol	Chemical		is not transfered to					apoA-I	GP				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_45_2_287_s_8	14617740	A mutant form of ABCA1 (W590S) that avidly binds apoA-I but fails to promote cholesterol efflux released apoA-I with similar kinetics but without transfer of cholesterol to apoA-I.	bind
44427	5	11204	5	10	NULL	NULL	NULL	statement 3	Process		occurs simultaneously with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_45_2_287_s_8	14617740	A mutant form of ABCA1 (W590S) that avidly binds apoA-I but fails to promote cholesterol efflux released apoA-I with similar kinetics but without transfer of cholesterol to apoA-I.	bind
44339	1	11204	6	10	NULL	NULL	NULL	ABCA1	GP	mutant	bind		avidly	W590S		apoA-I	GP				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_45_2_287_s_8	14617740	A mutant form of ABCA1 (W590S) that avidly binds apoA-I but fails to promote cholesterol efflux released apoA-I with similar kinetics but without transfer of cholesterol to apoA-I.	bind
44340	2	11204	6	10	NULL	NULL	NULL	ABCA1	GP	mutant	does not promote			W590S		cholesterol efflux	Process				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_45_2_287_s_8	14617740	A mutant form of ABCA1 (W590S) that avidly binds apoA-I but fails to promote cholesterol efflux released apoA-I with similar kinetics but without transfer of cholesterol to apoA-I.	bind
44999	3	11204	6	10	NULL	NULL	NULL	ABCA1	GP	mutant	releases			W590S		apoA-I	GP				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_45_2_287_s_8	14617740	A mutant form of ABCA1 (W590S) that avidly binds apoA-I but fails to promote cholesterol efflux released apoA-I with similar kinetics but without transfer of cholesterol to apoA-I.	bind
45000	4	11204	6	10	NULL	NULL	NULL	cholesterol	Chemical		is not transfered to					apoA-I	GP				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_45_2_287_s_8	14617740	A mutant form of ABCA1 (W590S) that avidly binds apoA-I but fails to promote cholesterol efflux released apoA-I with similar kinetics but without transfer of cholesterol to apoA-I.	bind
45002	5	11204	6	10	NULL	NULL	NULL	statement 3	Process		occurs simultaneous with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_45_2_287_s_8	14617740	A mutant form of ABCA1 (W590S) that avidly binds apoA-I but fails to promote cholesterol efflux released apoA-I with similar kinetics but without transfer of cholesterol to apoA-I.	bind
44483	1	11205	5	10	NULL	NULL	NULL	Armadillo	GP	mutant	lacks								fifth Armadillo repeat		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_4_181_s_222	9501980	A mutant form of Armadillo lacking the fifth Armadillo repeat fails to bind to  Drosophila TCF (and therefore lacks signaling activity), but accumulates in embryonic nuclei in response to Wingless (Wnt) signaling   [34,40]  .	bind
44484	2	11205	5	10	NULL	NULL	NULL	statement 1	GP		does not bind					TCF	GP	Drosophila			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_4_181_s_222	9501980	A mutant form of Armadillo lacking the fifth Armadillo repeat fails to bind to  Drosophila TCF (and therefore lacks signaling activity), but accumulates in embryonic nuclei in response to Wingless (Wnt) signaling   [34,40]  .	bind
44485	3	11205	5	10	NULL	NULL	NULL	statement 1	GP		lacks					signaling activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_4_181_s_222	9501980	A mutant form of Armadillo lacking the fifth Armadillo repeat fails to bind to  Drosophila TCF (and therefore lacks signaling activity), but accumulates in embryonic nuclei in response to Wingless (Wnt) signaling   [34,40]  .	bind
44486	4	11205	5	10	NULL	NULL	NULL	statement 1	GP		accumulates in					nucleus	CellComponent	embryonic			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_4_181_s_222	9501980	A mutant form of Armadillo lacking the fifth Armadillo repeat fails to bind to  Drosophila TCF (and therefore lacks signaling activity), but accumulates in embryonic nuclei in response to Wingless (Wnt) signaling   [34,40]  .	bind
44487	5	11205	5	10	NULL	NULL	NULL	statement 4	Process		in response to					Wnt signaling	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_4_181_s_222	9501980	A mutant form of Armadillo lacking the fifth Armadillo repeat fails to bind to  Drosophila TCF (and therefore lacks signaling activity), but accumulates in embryonic nuclei in response to Wingless (Wnt) signaling   [34,40]  .	bind
44488	6	11205	5	10	NULL	NULL	NULL	Wnt signaling	Process		is					Wingless signaling	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_4_181_s_222	9501980	A mutant form of Armadillo lacking the fifth Armadillo repeat fails to bind to  Drosophila TCF (and therefore lacks signaling activity), but accumulates in embryonic nuclei in response to Wingless (Wnt) signaling   [34,40]  .	bind
44341	1	11205	6	10	NULL	NULL	NULL	Armadillo	GP	mutant;; lacking	does not bind			fifth repeat		TCF	GP	Drosophila			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_4_181_s_222	9501980	A mutant form of Armadillo lacking the fifth Armadillo repeat fails to bind to  Drosophila TCF (and therefore lacks signaling activity), but accumulates in embryonic nuclei in response to Wingless (Wnt) signaling   [34,40]  .	bind
44342	2	11205	6	10	NULL	NULL	NULL	Armadillo	GP	mutant;; lacking	accumulates in			fifth repeat		nuclei	CellComponent	embryonic			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_4_181_s_222	9501980	A mutant form of Armadillo lacking the fifth Armadillo repeat fails to bind to  Drosophila TCF (and therefore lacks signaling activity), but accumulates in embryonic nuclei in response to Wingless (Wnt) signaling   [34,40]  .	bind
44343	3	11205	6	10	NULL	NULL	NULL	statement 2	Process		occurs in response to					wnt signaling	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_4_181_s_222	9501980	A mutant form of Armadillo lacking the fifth Armadillo repeat fails to bind to  Drosophila TCF (and therefore lacks signaling activity), but accumulates in embryonic nuclei in response to Wingless (Wnt) signaling   [34,40]  .	bind
44344	4	11205	6	10	NULL	NULL	NULL	Wnt	GP		is					wingless	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_4_181_s_222	9501980	A mutant form of Armadillo lacking the fifth Armadillo repeat fails to bind to  Drosophila TCF (and therefore lacks signaling activity), but accumulates in embryonic nuclei in response to Wingless (Wnt) signaling   [34,40]  .	bind
44345	5	11205	6	10	NULL	NULL	NULL	Armadillo	GP	mutant;; lacking	lacks			fifth repeat		signaling activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_4_181_s_222	9501980	A mutant form of Armadillo lacking the fifth Armadillo repeat fails to bind to  Drosophila TCF (and therefore lacks signaling activity), but accumulates in embryonic nuclei in response to Wingless (Wnt) signaling   [34,40]  .	bind
44346	6	11205	6	10	NULL	NULL	NULL	statement 5	Process		is because of					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_4_181_s_222	9501980	A mutant form of Armadillo lacking the fifth Armadillo repeat fails to bind to  Drosophila TCF (and therefore lacks signaling activity), but accumulates in embryonic nuclei in response to Wingless (Wnt) signaling   [34,40]  .	bind
44489	1	11206	5	NULL	NULL	NULL	NULL	axin	GP	mutant	does not bind					GSK3beta	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_39037_s_251	11487578	A mutant form of axin that did not bind to GSK3beta nevertheless promoted the phosphorylation of APC fragments when coexpressed with them.	bind
44490	2	11206	5	NULL	NULL	NULL	NULL	axin	GP	mutant	promotes					APC fragments	AminoAcid	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_39037_s_251	11487578	A mutant form of axin that did not bind to GSK3beta nevertheless promoted the phosphorylation of APC fragments when coexpressed with them.	bind
44347	1	11206	6	NULL	NULL	0	NULL	axin	NULL	mutant	does not bind	NULL				GSK-3beta	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_39037_s_251	11487578	A mutant form of axin that did not bind to GSK3beta nevertheless promoted the phosphorylation of APC fragments when coexpressed with them.	bind
44348	2	11206	6	NULL	NULL	0	NULL	axin	NULL	mutant	promotes	NULL				APC fragments	NULL	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_39037_s_251	11487578	A mutant form of axin that did not bind to GSK3beta nevertheless promoted the phosphorylation of APC fragments when coexpressed with them.	bind
44491	1	11207	5	NULL	NULL	NULL	NULL	CBP	GP	mutant	contains							deletion in	p160 binding region (amino acids 2098 to 2163) 		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_1_39_s_48	11113179	A mutant form of CBP containing a deletion in the p160 binding region (amino acids 2098 to 2163) inhibited RAR-mediated transcription in microinjected cells ( 34).	bind
44492	2	11207	5	NULL	NULL	NULL	NULL	statement 1	Process		inhibit					transcription	Process				NULL	microinjected cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_1_39_s_48	11113179	A mutant form of CBP containing a deletion in the p160 binding region (amino acids 2098 to 2163) inhibited RAR-mediated transcription in microinjected cells ( 34).	bind
44493	3	11207	5	NULL	NULL	NULL	NULL	transcription	Process		mediated by					RAR	GP				NULL	microinjected cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_1_39_s_48	11113179	A mutant form of CBP containing a deletion in the p160 binding region (amino acids 2098 to 2163) inhibited RAR-mediated transcription in microinjected cells ( 34).	bind
45005	1	11207	6	10	NULL	0	NULL	RAR			mediates					transcription					NULL	microinjected cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_1_39_s_48	11113179	A mutant form of CBP containing a deletion in the p160 binding region (amino acids 2098 to 2163) inhibited RAR-mediated transcription in microinjected cells ( 34).	bind
45006	2	11207	6	10	NULL	0	NULL	CBP		mutant;; deletion of	inhibits			p160 binding region		statement 1					NULL	microinjected cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_1_39_s_48	11113179	A mutant form of CBP containing a deletion in the p160 binding region (amino acids 2098 to 2163) inhibited RAR-mediated transcription in microinjected cells ( 34).	bind
44495	1	11208	5	NULL	NULL	NULL	NULL	Importin alpha	GP	mutant	does not bind		efficiently	ED		NLS proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1526_s_118	15014441	A mutant form of Importin alpha that does not bind efficiently to NLS proteins, the ED mutant (  et al), did not change mobility in the presence of CKII and NLS peptides ( Supplementary Figure 1A).	bind
44349	1	11208	6	10	NULL	0	NULL	Importin alpha	NULL	mutant	does not bind	NULL	efficiently	ED		NLS proteins	NULL				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_7_1526_s_118	15014441	A mutant form of Importin alpha that does not bind efficiently to NLS proteins, the ED mutant (  et al), did not change mobility in the presence of CKII and NLS peptides ( Supplementary Figure 1A).	bind
44499	1	11209	5	NULL	NULL	NULL	NULL	NGF3T	GP		is a mutant of					NGF	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_38_23547_s_56	9295291	A mutant form of NGF (NGF3T) that does not bind p75NTR ( 21) was used to selectively activate TrkA and BDNF was used to selectively activate p75NTR.	bind
44500	2	11209	5	NULL	NULL	NULL	NULL	statement 1	Process		does not bind					p75NTR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_38_23547_s_56	9295291	A mutant form of NGF (NGF3T) that does not bind p75NTR ( 21) was used to selectively activate TrkA and BDNF was used to selectively activate p75NTR.	bind
44501	3	11209	5	NULL	NULL	NULL	NULL	statement 1	Process		activates		selectively			TrkA	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_38_23547_s_56	9295291	A mutant form of NGF (NGF3T) that does not bind p75NTR ( 21) was used to selectively activate TrkA and BDNF was used to selectively activate p75NTR.	bind
44502	4	11209	5	NULL	NULL	NULL	NULL	BDNF	GP		activates		selectively			p75NTR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_38_23547_s_56	9295291	A mutant form of NGF (NGF3T) that does not bind p75NTR ( 21) was used to selectively activate TrkA and BDNF was used to selectively activate p75NTR.	bind
44350	1	11209	6	10	NULL	0	NULL	NGF3T			is a mutant of					NGF					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_38_23547_s_56	9295291	A mutant form of NGF (NGF3T) that does not bind p75NTR ( 21) was used to selectively activate TrkA and BDNF was used to selectively activate p75NTR.	bind
44351	2	11209	6	NULL	NULL	0	NULL	NGF3T	NULL		does not bind	NULL				p75NTR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_38_23547_s_56	9295291	A mutant form of NGF (NGF3T) that does not bind p75NTR ( 21) was used to selectively activate TrkA and BDNF was used to selectively activate p75NTR.	bind
44352	3	11209	6	10	NULL	0	NULL	NGF3T			activate		selectively			TrkA					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_38_23547_s_56	9295291	A mutant form of NGF (NGF3T) that does not bind p75NTR ( 21) was used to selectively activate TrkA and BDNF was used to selectively activate p75NTR.	bind
44353	4	11209	6	NULL	NULL	0	NULL	BDNF	NULL		activates	NULL	selectively			p75NTR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_38_23547_s_56	9295291	A mutant form of NGF (NGF3T) that does not bind p75NTR ( 21) was used to selectively activate TrkA and BDNF was used to selectively activate p75NTR.	bind
44503	1	11210	5	NULL	NULL	NULL	NULL	NHERF	GP	mutant	does not bind					EGFR	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_12_5470_s_29	15469991	A mutant form of NHERF that does not bind EGFR also enhances EGFR down-regulation, supporting the conclusion that NHERF functions to retain EGFR at the cell surface.	bind
44504	2	11210	5	NULL	NULL	NULL	NULL	NHERF	GP	mutant	enhance					EGFR	GP	down-regulation of			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_12_5470_s_29	15469991	A mutant form of NHERF that does not bind EGFR also enhances EGFR down-regulation, supporting the conclusion that NHERF functions to retain EGFR at the cell surface.	bind
44505	3	11210	5	NULL	NULL	NULL	NULL	NHERF	GP		retains					EGFR	GP				NULL	cell surface	NULL	NULL	NULL	NULL	gw70_molbiolcell_15_12_5470_s_29	15469991	A mutant form of NHERF that does not bind EGFR also enhances EGFR down-regulation, supporting the conclusion that NHERF functions to retain EGFR at the cell surface.	bind
44354	1	11210	6	NULL	NULL	0	NULL	NHERF	NULL	mutant	does not bind	NULL				EGFR	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_12_5470_s_29	15469991	A mutant form of NHERF that does not bind EGFR also enhances EGFR down-regulation, supporting the conclusion that NHERF functions to retain EGFR at the cell surface.	bind
44355	2	11210	6	NULL	NULL	0	NULL	NHERF	NULL	mutant	enhances	NULL				EGFR	NULL	downregulation of			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_12_5470_s_29	15469991	A mutant form of NHERF that does not bind EGFR also enhances EGFR down-regulation, supporting the conclusion that NHERF functions to retain EGFR at the cell surface.	bind
44356	3	11210	6	10	NULL	0	NULL	NHERF			retains					EGFR					NULL	cell surface	NULL	NULL	NULL	NULL	gw70_molbiolcell_15_12_5470_s_29	15469991	A mutant form of NHERF that does not bind EGFR also enhances EGFR down-regulation, supporting the conclusion that NHERF functions to retain EGFR at the cell surface.	bind
44506	1	11211	5	NULL	NULL	NULL	NULL	p120 ctn	GP	mutant	does not bind					cadherins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_15_11264_s_10	10753936	A mutant form of p120 ctn that fails to bind cadherins can still associate with RPTPmu.	bind
44507	2	11211	5	NULL	NULL	NULL	NULL	statement 1	Process		associate with					RPTPmu	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_15_11264_s_10	10753936	A mutant form of p120 ctn that fails to bind cadherins can still associate with RPTPmu.	bind
44358	1	11211	6	NULL	NULL	0	NULL	p120 ctn	NULL	mutant	does not bind	NULL				cadherin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_15_11264_s_10	10753936	A mutant form of p120 ctn that fails to bind cadherins can still associate with RPTPmu.	bind
44359	2	11211	6	NULL	NULL	0	NULL	p120 ctn	NULL	mutant	associates with	NULL				RPTPmu	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_15_11264_s_10	10753936	A mutant form of p120 ctn that fails to bind cadherins can still associate with RPTPmu.	bind
44508	1	11213	5	NULL	NULL	NULL	NULL	Pyk2	GP	mutant	does not bind			Y402F		Src	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14893_s_218	10329689	A mutant form of Pyk2 (Pyk2-Y402F) that is unable to bind and activate Src is impaired in its ability to induce association of Grb2 with Shc, binding of Crk to p130Cas and stimulation of the ERK and JNK cascades.	bind
44509	2	11213	5	NULL	NULL	NULL	NULL	statement 1	Process		does not activate					Src	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14893_s_218	10329689	A mutant form of Pyk2 (Pyk2-Y402F) that is unable to bind and activate Src is impaired in its ability to induce association of Grb2 with Shc, binding of Crk to p130Cas and stimulation of the ERK and JNK cascades.	bind
44510	3	11213	5	NULL	NULL	NULL	NULL	Grb2	GP		associate with					Shc	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14893_s_218	10329689	A mutant form of Pyk2 (Pyk2-Y402F) that is unable to bind and activate Src is impaired in its ability to induce association of Grb2 with Shc, binding of Crk to p130Cas and stimulation of the ERK and JNK cascades.	bind
44511	4	11213	5	NULL	NULL	NULL	NULL	Pyk2	GP	mutant	does not induce			Y402F		statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14893_s_218	10329689	A mutant form of Pyk2 (Pyk2-Y402F) that is unable to bind and activate Src is impaired in its ability to induce association of Grb2 with Shc, binding of Crk to p130Cas and stimulation of the ERK and JNK cascades.	bind
44512	5	11213	5	NULL	NULL	NULL	NULL	Crk	GP		bind					p130Cas	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14893_s_218	10329689	A mutant form of Pyk2 (Pyk2-Y402F) that is unable to bind and activate Src is impaired in its ability to induce association of Grb2 with Shc, binding of Crk to p130Cas and stimulation of the ERK and JNK cascades.	bind
44513	6	11213	5	NULL	NULL	NULL	NULL	Pyk2	GP	mutant	does not induce			Y402F		statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14893_s_218	10329689	A mutant form of Pyk2 (Pyk2-Y402F) that is unable to bind and activate Src is impaired in its ability to induce association of Grb2 with Shc, binding of Crk to p130Cas and stimulation of the ERK and JNK cascades.	bind
44514	7	11213	5	NULL	NULL	NULL	NULL	Pyk2	GP	mutant	does not stimulate			Y402F		ERK cascade	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14893_s_218	10329689	A mutant form of Pyk2 (Pyk2-Y402F) that is unable to bind and activate Src is impaired in its ability to induce association of Grb2 with Shc, binding of Crk to p130Cas and stimulation of the ERK and JNK cascades.	bind
44515	8	11213	5	NULL	NULL	NULL	NULL	Pyk2	GP	mutant	does not stimulate			Y402F		JNK cascade	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14893_s_218	10329689	A mutant form of Pyk2 (Pyk2-Y402F) that is unable to bind and activate Src is impaired in its ability to induce association of Grb2 with Shc, binding of Crk to p130Cas and stimulation of the ERK and JNK cascades.	bind
44442	1	11213	6	NULL	NULL	0	NULL	Pyk2	NULL	mutant	does not bind	NULL		Y402F		Src	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_21_14893_s_218	10329689	A mutant form of Pyk2 (Pyk2-Y402F) that is unable to bind and activate Src is impaired in its ability to induce association of Grb2 with Shc, binding of Crk to p130Cas and stimulation of the ERK and JNK cascades.	bind
44443	2	11213	6	NULL	NULL	0	NULL	Pyk2	NULL	mutant	does not activate	NULL		Y402F		Src	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_21_14893_s_218	10329689	A mutant form of Pyk2 (Pyk2-Y402F) that is unable to bind and activate Src is impaired in its ability to induce association of Grb2 with Shc, binding of Crk to p130Cas and stimulation of the ERK and JNK cascades.	bind
44444	3	11213	6	NULL	NULL	0	NULL	Grb2	NULL		associates with	NULL				Shc	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_21_14893_s_218	10329689	A mutant form of Pyk2 (Pyk2-Y402F) that is unable to bind and activate Src is impaired in its ability to induce association of Grb2 with Shc, binding of Crk to p130Cas and stimulation of the ERK and JNK cascades.	bind
44445	4	11213	6	NULL	NULL	0	NULL	Pyk2	NULL	mutant	does not induce	NULL		Y402F		statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_21_14893_s_218	10329689	A mutant form of Pyk2 (Pyk2-Y402F) that is unable to bind and activate Src is impaired in its ability to induce association of Grb2 with Shc, binding of Crk to p130Cas and stimulation of the ERK and JNK cascades.	bind
44446	5	11213	6	NULL	NULL	0	NULL	Crk	NULL		bind	NULL				p130Cas	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_21_14893_s_218	10329689	A mutant form of Pyk2 (Pyk2-Y402F) that is unable to bind and activate Src is impaired in its ability to induce association of Grb2 with Shc, binding of Crk to p130Cas and stimulation of the ERK and JNK cascades.	bind
44447	6	11213	6	NULL	NULL	0	NULL	Pyk2	NULL	mutant	does not induce	NULL		Y402F		statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_21_14893_s_218	10329689	A mutant form of Pyk2 (Pyk2-Y402F) that is unable to bind and activate Src is impaired in its ability to induce association of Grb2 with Shc, binding of Crk to p130Cas and stimulation of the ERK and JNK cascades.	bind
44448	7	11213	6	NULL	NULL	0	NULL	Pyk2	NULL	mutant	does not induce	NULL		Y402F		ERK cascade	NULL	stimulation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_21_14893_s_218	10329689	A mutant form of Pyk2 (Pyk2-Y402F) that is unable to bind and activate Src is impaired in its ability to induce association of Grb2 with Shc, binding of Crk to p130Cas and stimulation of the ERK and JNK cascades.	bind
44449	8	11213	6	NULL	NULL	0	NULL	Pyk2	NULL	mutant	does not induce	NULL		Y402F		JNK cascade	NULL	stimulation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_21_14893_s_218	10329689	A mutant form of Pyk2 (Pyk2-Y402F) that is unable to bind and activate Src is impaired in its ability to induce association of Grb2 with Shc, binding of Crk to p130Cas and stimulation of the ERK and JNK cascades.	bind
44516	1	11214	5	NULL	NULL	NULL	NULL	deltap85	GP		is a mutant of					PI3-K	GP		p85 regulatory subunit		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31515_s_145	9395488	A mutant form of the p85 regulatory subunit of PI3-K (deltap85) that fails to bind and activate the p110 catalytic subunit has been reported to act as a dominant negative mutant of this enzyme ( 34) and to abolish platelet-derived growth factor-induced activation of PKB in cotransfection experiments ( 5).	bind
44517	2	11214	5	NULL	NULL	NULL	NULL	deltap85 	GP		does not bind					p110	GP		catalytic subunit		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31515_s_145	9395488	A mutant form of the p85 regulatory subunit of PI3-K (deltap85) that fails to bind and activate the p110 catalytic subunit has been reported to act as a dominant negative mutant of this enzyme ( 34) and to abolish platelet-derived growth factor-induced activation of PKB in cotransfection experiments ( 5).	bind
44518	3	11214	5	NULL	NULL	NULL	NULL	deltap85	GP		does not activate					p110	GP		catalytic subunit		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31515_s_145	9395488	A mutant form of the p85 regulatory subunit of PI3-K (deltap85) that fails to bind and activate the p110 catalytic subunit has been reported to act as a dominant negative mutant of this enzyme ( 34) and to abolish platelet-derived growth factor-induced activation of PKB in cotransfection experiments ( 5).	bind
44519	4	11214	5	NULL	NULL	NULL	NULL	deltap85	GP		acts as					PI3-K	GP	dominant negative mutant of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31515_s_145	9395488	A mutant form of the p85 regulatory subunit of PI3-K (deltap85) that fails to bind and activate the p110 catalytic subunit has been reported to act as a dominant negative mutant of this enzyme ( 34) and to abolish platelet-derived growth factor-induced activation of PKB in cotransfection experiments ( 5).	bind
44520	5	11214	5	NULL	NULL	NULL	NULL	platelet-derived growth factor	GP		induce					PKB	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31515_s_145	9395488	A mutant form of the p85 regulatory subunit of PI3-K (deltap85) that fails to bind and activate the p110 catalytic subunit has been reported to act as a dominant negative mutant of this enzyme ( 34) and to abolish platelet-derived growth factor-induced activation of PKB in cotransfection experiments ( 5).	bind
44521	6	11214	5	NULL	NULL	NULL	NULL	deltap85	GP		abolishes					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31515_s_145	9395488	A mutant form of the p85 regulatory subunit of PI3-K (deltap85) that fails to bind and activate the p110 catalytic subunit has been reported to act as a dominant negative mutant of this enzyme ( 34) and to abolish platelet-derived growth factor-induced activation of PKB in cotransfection experiments ( 5).	bind
44450	1	11214	6	10	NULL	0	NULL	deltap85			is a mutant of					PI3-K			p85 regulatory subunit		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31515_s_145	9395488	A mutant form of the p85 regulatory subunit of PI3-K (deltap85) that fails to bind and activate the p110 catalytic subunit has been reported to act as a dominant negative mutant of this enzyme ( 34) and to abolish platelet-derived growth factor-induced activation of PKB in cotransfection experiments ( 5).	bind
44451	2	11214	6	10	NULL	0	NULL	deltap85			does not bind					p110			catalytic subunit		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31515_s_145	9395488	A mutant form of the p85 regulatory subunit of PI3-K (deltap85) that fails to bind and activate the p110 catalytic subunit has been reported to act as a dominant negative mutant of this enzyme ( 34) and to abolish platelet-derived growth factor-induced activation of PKB in cotransfection experiments ( 5).	bind
44452	3	11214	6	10	NULL	0	NULL	platelet-derived growth factor			induces					PKB		activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31515_s_145	9395488	A mutant form of the p85 regulatory subunit of PI3-K (deltap85) that fails to bind and activate the p110 catalytic subunit has been reported to act as a dominant negative mutant of this enzyme ( 34) and to abolish platelet-derived growth factor-induced activation of PKB in cotransfection experiments ( 5).	bind
44453	4	11214	6	10	NULL	0	NULL	deltap85			abolishes					statement 3					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_50_31515_s_145	9395488	A mutant form of the p85 regulatory subunit of PI3-K (deltap85) that fails to bind and activate the p110 catalytic subunit has been reported to act as a dominant negative mutant of this enzyme ( 34) and to abolish platelet-derived growth factor-induced activation of PKB in cotransfection experiments ( 5).	bind
50855	5	11214	6	10	NULL	0	NULL	deltap85	NULL		does not activate	NULL				p110	NULL		catalytic subuni		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_50_31515_s_145	9395488	A mutant form of the p85 regulatory subunit of PI3-K (deltap85) that fails to bind and activate the p110 catalytic subunit has been reported to act as a dominant negative mutant of this enzyme ( 34) and to abolish platelet-derived growth factor-induced activation of PKB in cotransfection experiments ( 5).	bind
50856	6	11214	6	10	NULL	0	NULL	deltap85	NULL		acts as	NULL				PI3-K	NULL	 dominant negative mutant of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_50_31515_s_145	9395488	A mutant form of the p85 regulatory subunit of PI3-K (deltap85) that fails to bind and activate the p110 catalytic subunit has been reported to act as a dominant negative mutant of this enzyme ( 34) and to abolish platelet-derived growth factor-induced activation of PKB in cotransfection experiments ( 5).	bind
44522	1	11216	5	NULL	NULL	NULL	NULL	Cyclin A1	GP		is a mutant of			E167A		Cyclin A1	GP		N-terminal Helix		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_15415_s_169	11278837	A Mutant in the N-terminal Helix of Cyclin A1, E167A, Can Bind to Cdc2 But Not to Cdk2-- Cyclin A binds to both Cdc2 and Cdk2.	bind
44523	2	11216	5	NULL	NULL	NULL	NULL	statement 1	Process		bind					Cdc2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_15415_s_169	11278837	A Mutant in the N-terminal Helix of Cyclin A1, E167A, Can Bind to Cdc2 But Not to Cdk2-- Cyclin A binds to both Cdc2 and Cdk2.	bind
44524	3	11216	5	NULL	NULL	NULL	NULL	statement 1	Process		does not bind					Cdk2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_15415_s_169	11278837	A Mutant in the N-terminal Helix of Cyclin A1, E167A, Can Bind to Cdc2 But Not to Cdk2-- Cyclin A binds to both Cdc2 and Cdk2.	bind
44525	4	11216	5	NULL	NULL	NULL	NULL	Cyclin A	GP		bind					Cdc2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_15415_s_169	11278837	A Mutant in the N-terminal Helix of Cyclin A1, E167A, Can Bind to Cdc2 But Not to Cdk2-- Cyclin A binds to both Cdc2 and Cdk2.	bind
44526	5	11216	5	NULL	NULL	NULL	NULL	Cyclin A	GP		bind					Cdk2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_15415_s_169	11278837	A Mutant in the N-terminal Helix of Cyclin A1, E167A, Can Bind to Cdc2 But Not to Cdk2-- Cyclin A binds to both Cdc2 and Cdk2.	bind
44454	1	11216	6	NULL	NULL	0	NULL	Cyclin A1	NULL	mutant	bind	NULL		N-terminal helix;; E167A		Cdc2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_15415_s_169	11278837	A Mutant in the N-terminal Helix of Cyclin A1, E167A, Can Bind to Cdc2 But Not to Cdk2-- Cyclin A binds to both Cdc2 and Cdk2.	bind
44455	2	11216	6	10	NULL	0	NULL	Cyclin A1	NULL	mutant	does not bind	NULL		N-terminal helix;; E167A		Cdk2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_15415_s_169	11278837	A Mutant in the N-terminal Helix of Cyclin A1, E167A, Can Bind to Cdc2 But Not to Cdk2-- Cyclin A binds to both Cdc2 and Cdk2.	bind
44456	3	11216	6	10	NULL	0	NULL	Cyclin A	NULL		bind	NULL				Cdc2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_15415_s_169	11278837	A Mutant in the N-terminal Helix of Cyclin A1, E167A, Can Bind to Cdc2 But Not to Cdk2-- Cyclin A binds to both Cdc2 and Cdk2.	bind
50857	4	11216	6	10	NULL	0	NULL	Cyclin A	NULL		bind	NULL				Cdk2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_18_15415_s_169	11278837	A Mutant in the N-terminal Helix of Cyclin A1, E167A, Can Bind to Cdc2 But Not to Cdk2-- Cyclin A binds to both Cdc2 and Cdk2.	bind
44527	1	11217	5	NULL	NULL	NULL	NULL	ATF6	GP	mutant of	lacks			468-500					GLSs		NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_1_99_s_218	12110171	A mutant lacking the GLSs, ATF6( 468-500), bound and dissociated from BiP like wild-type ATF6   (Figure 5D).	bind
44528	2	11217	5	NULL	NULL	NULL	NULL	statement 1	Process		dissociates from					BiP	GP	wild-type			NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_1_99_s_218	12110171	A mutant lacking the GLSs, ATF6( 468-500), bound and dissociated from BiP like wild-type ATF6   (Figure 5D).	bind
46365	3	11217	5	NULL	NULL	NULL	NULL	ATF6	GP	wild-type	bind					BiP	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_1_99_s_218	12110171	A mutant lacking the GLSs, ATF6( 468-500), bound and dissociated from BiP like wild-type ATF6   (Figure 5D).	bind
46366	4	11217	5	NULL	NULL	NULL	NULL	statement 1	Process		is similar to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_1_99_s_218	12110171	A mutant lacking the GLSs, ATF6( 468-500), bound and dissociated from BiP like wild-type ATF6   (Figure 5D).	bind
46367	5	11217	5	NULL	NULL	NULL	NULL	ATF6	GP	wild type	dissociates from					BiP	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_1_99_s_218	12110171	A mutant lacking the GLSs, ATF6( 468-500), bound and dissociated from BiP like wild-type ATF6   (Figure 5D).	bind
46368	6	11217	5	NULL	NULL	NULL	NULL	ATF6	GP	mutation of	dissociates from			468-500		BiP	GP				NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_1_99_s_218	12110171	A mutant lacking the GLSs, ATF6( 468-500), bound and dissociated from BiP like wild-type ATF6   (Figure 5D).	bind
46369	7	11217	5	NULL	NULL	NULL	NULL	statement 5	Process		is similar to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_1_99_s_218	12110171	A mutant lacking the GLSs, ATF6( 468-500), bound and dissociated from BiP like wild-type ATF6   (Figure 5D).	bind
44457	1	11217	6	NULL	NULL	0	NULL	ATF6	NULL	wild type	bind	NULL				BiP	NULL				NULL		0	NULL	NULL	NULL	gw60_devcell_3_1_99_s_218	12110171	A mutant lacking the GLSs, ATF6( 468-500), bound and dissociated from BiP like wild-type ATF6   (Figure 5D).	bind
44458	2	11217	6	NULL	NULL	0	NULL	ATF6	NULL	mutant of 	bind	NULL		468-500		BiP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_1_99_s_218	12110171	A mutant lacking the GLSs, ATF6( 468-500), bound and dissociated from BiP like wild-type ATF6   (Figure 5D).	bind
46354	3	11217	6	NULL	NULL	0	NULL	statement 1	NULL		is similar to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_devcell_3_1_99_s_218	12110171	A mutant lacking the GLSs, ATF6( 468-500), bound and dissociated from BiP like wild-type ATF6   (Figure 5D).	bind
46355	4	11217	6	NULL	NULL	0	NULL	ATF6	NULL	wild type	dissociates from	NULL				BiP	NULL				NULL		0	NULL	NULL	NULL	gw60_devcell_3_1_99_s_218	12110171	A mutant lacking the GLSs, ATF6( 468-500), bound and dissociated from BiP like wild-type ATF6   (Figure 5D).	bind
46356	5	11217	6	NULL	NULL	0	NULL	ATF6	NULL	mutant of	dissociates from	NULL		468-500		BiP	NULL				NULL		0	NULL	NULL	NULL	gw60_devcell_3_1_99_s_218	12110171	A mutant lacking the GLSs, ATF6( 468-500), bound and dissociated from BiP like wild-type ATF6   (Figure 5D).	bind
46357	6	11217	6	NULL	NULL	0	NULL	statement 4	NULL		is similar to	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_devcell_3_1_99_s_218	12110171	A mutant lacking the GLSs, ATF6( 468-500), bound and dissociated from BiP like wild-type ATF6   (Figure 5D).	bind
50858	7	11217	6	10	NULL	0	NULL	ATF6	NULL	mutant	lacks	NULL		468-500		GLSs	NULL				NULL		NULL	NULL	NULL	NULL	gw60_devcell_3_1_99_s_218	12110171	A mutant lacking the GLSs, ATF6( 468-500), bound and dissociated from BiP like wild-type ATF6   (Figure 5D).	bind
44627	1	11218	5	NULL	NULL	NULL	NULL			mutant	lacks					Fe(III) resistance genes	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803591_s_8	16803591	A mutant lacking the PmrA-regulated  Fe(III) resistance genes bound more Fe(III) than the wild-type strain  and was defective for survival in soil, suggesting that these PmrA-regulated  lipopolysaccharide modifications aid Salmonella's survival and spread  in non-host environments.	bind
44628	2	11218	5	NULL	NULL	NULL	NULL	Fe(III) resistance genes	GP		is regulated by					PmrA	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803591_s_8	16803591	A mutant lacking the PmrA-regulated  Fe(III) resistance genes bound more Fe(III) than the wild-type strain  and was defective for survival in soil, suggesting that these PmrA-regulated  lipopolysaccharide modifications aid Salmonella's survival and spread  in non-host environments.	bind
44629	3	11218	5	NULL	NULL	NULL	NULL	statement 1	Process		bind					Fe(III)	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803591_s_8	16803591	A mutant lacking the PmrA-regulated  Fe(III) resistance genes bound more Fe(III) than the wild-type strain  and was defective for survival in soil, suggesting that these PmrA-regulated  lipopolysaccharide modifications aid Salmonella's survival and spread  in non-host environments.	bind
44630	4	11218	5	NULL	NULL	NULL	NULL	strain		wild-type	bind					Fe(III)	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803591_s_8	16803591	A mutant lacking the PmrA-regulated  Fe(III) resistance genes bound more Fe(III) than the wild-type strain  and was defective for survival in soil, suggesting that these PmrA-regulated  lipopolysaccharide modifications aid Salmonella's survival and spread  in non-host environments.	bind
44631	5	11218	5	NULL	NULL	NULL	NULL	statement 3	Process	binding of	is more than					statement 4	Process	binding of			NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803591_s_8	16803591	A mutant lacking the PmrA-regulated  Fe(III) resistance genes bound more Fe(III) than the wild-type strain  and was defective for survival in soil, suggesting that these PmrA-regulated  lipopolysaccharide modifications aid Salmonella's survival and spread  in non-host environments.	bind
44632	6	11218	5	NULL	NULL	NULL	NULL	statement 1	Process		does not survive in					soil	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803591_s_8	16803591	A mutant lacking the PmrA-regulated  Fe(III) resistance genes bound more Fe(III) than the wild-type strain  and was defective for survival in soil, suggesting that these PmrA-regulated  lipopolysaccharide modifications aid Salmonella's survival and spread  in non-host environments.	bind
44633	7	11218	5	NULL	NULL	NULL	NULL	lipopolysaccharide	Chemical	modifications of	aid in					Salmonella	Organism	survival of			NULL	non-host environments	NULL	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803591_s_8	16803591	A mutant lacking the PmrA-regulated  Fe(III) resistance genes bound more Fe(III) than the wild-type strain  and was defective for survival in soil, suggesting that these PmrA-regulated  lipopolysaccharide modifications aid Salmonella's survival and spread  in non-host environments.	bind
44634	8	11218	5	NULL	NULL	NULL	NULL	lipopolysaccharide	Chemical	modifications of	aid in					Salmonella	Organism	spreading of			NULL	non-host environments	NULL	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803591_s_8	16803591	A mutant lacking the PmrA-regulated  Fe(III) resistance genes bound more Fe(III) than the wild-type strain  and was defective for survival in soil, suggesting that these PmrA-regulated  lipopolysaccharide modifications aid Salmonella's survival and spread  in non-host environments.	bind
44635	9	11218	5	NULL	NULL	NULL	NULL	lipopolysaccharide	Chemical	modifications of	is regulated by					PmrA	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803591_s_8	16803591	A mutant lacking the PmrA-regulated  Fe(III) resistance genes bound more Fe(III) than the wild-type strain  and was defective for survival in soil, suggesting that these PmrA-regulated  lipopolysaccharide modifications aid Salmonella's survival and spread  in non-host environments.	bind
45008	1	11218	6	10	NULL	0	NULL	PmrA	NULL		regulates	NULL				Fe(III) resistance gene	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803591_s_8	16803591	A mutant lacking the PmrA-regulated  Fe(III) resistance genes bound more Fe(III) than the wild-type strain  and was defective for survival in soil, suggesting that these PmrA-regulated  lipopolysaccharide modifications aid Salmonella's survival and spread  in non-host environments.	bind
45009	2	11218	6	10	NULL	0	NULL		NULL	mutant	lacks	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803591_s_8	16803591	A mutant lacking the PmrA-regulated  Fe(III) resistance genes bound more Fe(III) than the wild-type strain  and was defective for survival in soil, suggesting that these PmrA-regulated  lipopolysaccharide modifications aid Salmonella's survival and spread  in non-host environments.	bind
45010	4	11218	6	10	NULL	0	NULL	strain	NULL	wild-type	bind	NULL				Fe(III)	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803591_s_8	16803591	A mutant lacking the PmrA-regulated  Fe(III) resistance genes bound more Fe(III) than the wild-type strain  and was defective for survival in soil, suggesting that these PmrA-regulated  lipopolysaccharide modifications aid Salmonella's survival and spread  in non-host environments.	bind
45011	5	11218	6	10	NULL	0	NULL	PmrA	NULL		regulates	NULL				lipopolysaccharide	NULL	modification of 			NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803591_s_8	16803591	A mutant lacking the PmrA-regulated  Fe(III) resistance genes bound more Fe(III) than the wild-type strain  and was defective for survival in soil, suggesting that these PmrA-regulated  lipopolysaccharide modifications aid Salmonella's survival and spread  in non-host environments.	bind
45012	7	11218	6	10	NULL	0	NULL	statement 5	NULL		aids in	NULL				cell survival	NULL	salmonella			NULL	non-host environments	NULL	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803591_s_8	16803591	A mutant lacking the PmrA-regulated  Fe(III) resistance genes bound more Fe(III) than the wild-type strain  and was defective for survival in soil, suggesting that these PmrA-regulated  lipopolysaccharide modifications aid Salmonella's survival and spread  in non-host environments.	bind
51052	6	11218	6	10	NULL	0	NULL	statement 3	NULL	binding of	is more than	NULL				statement 4	NULL	binding of			NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803591_s_8	16803591	A mutant lacking the PmrA-regulated  Fe(III) resistance genes bound more Fe(III) than the wild-type strain  and was defective for survival in soil, suggesting that these PmrA-regulated  lipopolysaccharide modifications aid Salmonella's survival and spread  in non-host environments.	bind
51053	3	11218	6	10	NULL	0	NULL	statement 2	NULL		bind	NULL				Fe(III)	NULL				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803591_s_8	16803591	A mutant lacking the PmrA-regulated  Fe(III) resistance genes bound more Fe(III) than the wild-type strain  and was defective for survival in soil, suggesting that these PmrA-regulated  lipopolysaccharide modifications aid Salmonella's survival and spread  in non-host environments.	bind
51054	8	11218	6	10	NULL	0	NULL	statement 5	NULL		aid in 	NULL				Salmonella	NULL	spreading of			NULL	non-host environments	0	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803591_s_8	16803591	A mutant lacking the PmrA-regulated  Fe(III) resistance genes bound more Fe(III) than the wild-type strain  and was defective for survival in soil, suggesting that these PmrA-regulated  lipopolysaccharide modifications aid Salmonella's survival and spread  in non-host environments.	bind
44529	1	11219	5	NULL	NULL	NULL	NULL	estrogen receptor	GP	mutant	bind			LBD		tamoxifen	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_36_0_687_s_444	12429705	A mutant ligand-binding domain of the estrogen receptor (LBD), which binds tamoxifen  instead of estrogen ( 68), was fused to a dominant-negative CREB gene (S133A substitution).	bind
44530	2	11219	5	NULL	NULL	NULL	NULL	LBD	AminoAcid		is					ligand-binding domain	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_36_0_687_s_444	12429705	A mutant ligand-binding domain of the estrogen receptor (LBD), which binds tamoxifen  instead of estrogen ( 68), was fused to a dominant-negative CREB gene (S133A substitution).	bind
44459	1	11219	6	10	NULL	0	NULL	estrogen receptor		mutant	bind			LBD		tamoxifen					NULL		NULL	NULL	NULL	NULL	gw70_annurevgenet_36_0_687_s_444	12429705	A mutant ligand-binding domain of the estrogen receptor (LBD), which binds tamoxifen  instead of estrogen ( 68), was fused to a dominant-negative CREB gene (S133A substitution).	bind
44460	2	11219	6	NULL	NULL	0	NULL	LBD	NULL		is	NULL				ligand binding domain	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevgenet_36_0_687_s_444	12429705	A mutant ligand-binding domain of the estrogen receptor (LBD), which binds tamoxifen  instead of estrogen ( 68), was fused to a dominant-negative CREB gene (S133A substitution).	bind
44531	1	11220	5	NULL	NULL	NULL	NULL	mDab555	GP	mutant	is changed to			Tyr198		mDab555	GP	mutant	Phe		NULL		NULL	NULL	NULL	NULL	gw60_embo_16_1_121_s_173	9009273	A mutant mDab555, in which Tyr198 and 200 were both changed to Phe, was phosphorylated on tyrosine to a reduced extent when co-expressed with Src527F, and bound to the Src SH2 domain  in vitro (Figure  5A).	bind
44532	2	11220	5	NULL	NULL	NULL	NULL	mDab555	GP	mutant	is changed to			Tyr200		mDab555	GP	mutant	Phe		NULL		NULL	NULL	NULL	NULL	gw60_embo_16_1_121_s_173	9009273	A mutant mDab555, in which Tyr198 and 200 were both changed to Phe, was phosphorylated on tyrosine to a reduced extent when co-expressed with Src527F, and bound to the Src SH2 domain  in vitro (Figure  5A).	bind
44533	3	11220	5	NULL	NULL	NULL	NULL	Src	GP		phosphorylate		weakly	527F		statement 1	Process		tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_embo_16_1_121_s_173	9009273	A mutant mDab555, in which Tyr198 and 200 were both changed to Phe, was phosphorylated on tyrosine to a reduced extent when co-expressed with Src527F, and bound to the Src SH2 domain  in vitro (Figure  5A).	bind
44534	4	11220	5	NULL	NULL	NULL	NULL	Src	GP		phosphorylate		weakly	527F		statement 2	Process		tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_embo_16_1_121_s_173	9009273	A mutant mDab555, in which Tyr198 and 200 were both changed to Phe, was phosphorylated on tyrosine to a reduced extent when co-expressed with Src527F, and bound to the Src SH2 domain  in vitro (Figure  5A).	bind
44536	5	11220	5	NULL	NULL	NULL	NULL	statement 1	Process		bind					Src	GP		SH2 domain		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_16_1_121_s_173	9009273	A mutant mDab555, in which Tyr198 and 200 were both changed to Phe, was phosphorylated on tyrosine to a reduced extent when co-expressed with Src527F, and bound to the Src SH2 domain  in vitro (Figure  5A).	bind
44537	6	11220	5	NULL	NULL	NULL	NULL	statement 2	Process		bind					Src	GP		SH2 domain		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_16_1_121_s_173	9009273	A mutant mDab555, in which Tyr198 and 200 were both changed to Phe, was phosphorylated on tyrosine to a reduced extent when co-expressed with Src527F, and bound to the Src SH2 domain  in vitro (Figure  5A).	bind
45013	1	11220	6	10	NULL	0	NULL	mDab555		mutant	is changed to			Tyr198		mDab555		mutant	Phe		NULL		NULL	NULL	NULL	NULL	gw60_embo_16_1_121_s_173	9009273	A mutant mDab555, in which Tyr198 and 200 were both changed to Phe, was phosphorylated on tyrosine to a reduced extent when co-expressed with Src527F, and bound to the Src SH2 domain  in vitro (Figure  5A).	bind
45014	2	11220	6	10	NULL	0	NULL	mDab555		mutant	is changed to			Tyr200		mDab555		mutant	Phe		NULL		NULL	NULL	NULL	NULL	gw60_embo_16_1_121_s_173	9009273	A mutant mDab555, in which Tyr198 and 200 were both changed to Phe, was phosphorylated on tyrosine to a reduced extent when co-expressed with Src527F, and bound to the Src SH2 domain  in vitro (Figure  5A).	bind
45015	3	11220	6	10	NULL	0	NULL	statement 1	NULL		bind	NULL				Src	NULL		SH2 domain		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_16_1_121_s_173	9009273	A mutant mDab555, in which Tyr198 and 200 were both changed to Phe, was phosphorylated on tyrosine to a reduced extent when co-expressed with Src527F, and bound to the Src SH2 domain  in vitro (Figure  5A).	bind
51207	4	11220	6	10	NULL	0	NULL	statement 2			bind					Src			SH2 domain		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_embo_16_1_121_s_173	9009273	A mutant mDab555, in which Tyr198 and 200 were both changed to Phe, was phosphorylated on tyrosine to a reduced extent when co-expressed with Src527F, and bound to the Src SH2 domain  in vitro (Figure  5A).	bind
44541	1	11221	5	NULL	NULL	NULL	NULL	EbpS	GP	mutant;;S. aureus	bind					tropoelastin	GP	radiolabeled			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_1_243_s_41	11684686	A mutant of  S. aureus lacking EbpS exhibited decreased binding to radiolabeled tropoelastin, a defect that was restored by the presence of the wild-type  ebpS gene on a complementing plasmid.	bind
44542	2	11221	5	NULL	NULL	NULL	NULL	EbpS	GP	wild-type;;S. aureus	bind					tropoelastin	GP	radiolabeled			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_1_243_s_41	11684686	A mutant of  S. aureus lacking EbpS exhibited decreased binding to radiolabeled tropoelastin, a defect that was restored by the presence of the wild-type  ebpS gene on a complementing plasmid.	bind
60504	3	11221	5	NULL	NULL	NULL	NULL	statement 2	Process		lesser than					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_1_243_s_41	11684686	A mutant of  S. aureus lacking EbpS exhibited decreased binding to radiolabeled tropoelastin, a defect that was restored by the presence of the wild-type  ebpS gene on a complementing plasmid.	bind
44462	1	11221	6	NULL	NULL	0	NULL	EbpS	NULL	S.aureus;; mutant	bind	NULL				tropoelastin	NULL	radiolabeled			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_1_243_s_41	11684686	A mutant of  S. aureus lacking EbpS exhibited decreased binding to radiolabeled tropoelastin, a defect that was restored by the presence of the wild-type  ebpS gene on a complementing plasmid.	bind
44463	2	11221	6	10	NULL	0	NULL	EbpS	NULL	S.aureus;;wild-type	bind	NULL				tropoelastin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_1_243_s_41	11684686	A mutant of  S. aureus lacking EbpS exhibited decreased binding to radiolabeled tropoelastin, a defect that was restored by the presence of the wild-type  ebpS gene on a complementing plasmid.	bind
44464	3	11221	6	NULL	NULL	0	NULL	statement 2	NULL		is less than	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_1_243_s_41	11684686	A mutant of  S. aureus lacking EbpS exhibited decreased binding to radiolabeled tropoelastin, a defect that was restored by the presence of the wild-type  ebpS gene on a complementing plasmid.	bind
44543	1	11222	5	NULL	NULL	NULL	NULL	DSC1	GP	component of;;mutant	affect					cdt2+	GP	expression of			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_genetics_164_3_881_s_5	12871901	A mutant of a component of DSC1 affected  cdt2+ expression  in vivo, and a  cdt2+ promoter fragment containing MCB motifs bound DSC1  in vitro.	bind
44544	2	11222	5	NULL	NULL	NULL	NULL	cdt2+	GP		contains				promoter fragment					MCB motifs	NULL		NULL	NULL	NULL	NULL	gw60_genetics_164_3_881_s_5	12871901	A mutant of a component of DSC1 affected  cdt2+ expression  in vivo, and a  cdt2+ promoter fragment containing MCB motifs bound DSC1  in vitro.	bind
44545	3	11222	5	NULL	NULL	NULL	NULL	statement 2	Process		bind					DSC1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_genetics_164_3_881_s_5	12871901	A mutant of a component of DSC1 affected  cdt2+ expression  in vivo, and a  cdt2+ promoter fragment containing MCB motifs bound DSC1  in vitro.	bind
44465	1	11222	6	NULL	NULL	0	NULL	DSC1	NULL	mutant	affects	NULL				cdt2+	NULL	expression of			NULL	in vivo	0	NULL	NULL	NULL	gw60_genetics_164_3_881_s_5	12871901	A mutant of a component of DSC1 affected  cdt2+ expression  in vivo, and a  cdt2+ promoter fragment containing MCB motifs bound DSC1  in vitro.	bind
44466	2	11222	6	NULL	NULL	0	NULL	cdt2+	NULL		bind	NULL		MCB motif	promoter	DSC1	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_genetics_164_3_881_s_5	12871901	A mutant of a component of DSC1 affected  cdt2+ expression  in vivo, and a  cdt2+ promoter fragment containing MCB motifs bound DSC1  in vitro.	bind
44546	1	11223	5	NULL	NULL	NULL	NULL	E1A	GP	mutant	bind					Stat1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_27_20406_s_183	10764778	A mutant of E1A that binds to Stat1 but not to CBP/p300 also down-regulates LMP2 transcription, whereas delta2-36, which binds to neither CBP/p300 nor Stat1, has no effect on the levels of LMP2 RNA in either U3A-701 or 2fTGH cells.	bind
44547	2	11223	5	NULL	NULL	NULL	NULL	E1A	GP	mutant	does not bind					CBP/p300	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_27_20406_s_183	10764778	A mutant of E1A that binds to Stat1 but not to CBP/p300 also down-regulates LMP2 transcription, whereas delta2-36, which binds to neither CBP/p300 nor Stat1, has no effect on the levels of LMP2 RNA in either U3A-701 or 2fTGH cells.	bind
44548	3	11223	5	NULL	NULL	NULL	NULL	E1A	GP	mutant	downregulates					LMP2	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_27_20406_s_183	10764778	A mutant of E1A that binds to Stat1 but not to CBP/p300 also down-regulates LMP2 transcription, whereas delta2-36, which binds to neither CBP/p300 nor Stat1, has no effect on the levels of LMP2 RNA in either U3A-701 or 2fTGH cells.	bind
44549	4	11223	5	NULL	NULL	NULL	NULL	delta2-36	GP		does not bind					CBP/p300	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_27_20406_s_183	10764778	A mutant of E1A that binds to Stat1 but not to CBP/p300 also down-regulates LMP2 transcription, whereas delta2-36, which binds to neither CBP/p300 nor Stat1, has no effect on the levels of LMP2 RNA in either U3A-701 or 2fTGH cells.	bind
44550	5	11223	5	NULL	NULL	NULL	NULL	delta2-36	GP		does not bind					Stat1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_27_20406_s_183	10764778	A mutant of E1A that binds to Stat1 but not to CBP/p300 also down-regulates LMP2 transcription, whereas delta2-36, which binds to neither CBP/p300 nor Stat1, has no effect on the levels of LMP2 RNA in either U3A-701 or 2fTGH cells.	bind
44551	6	11223	5	NULL	NULL	NULL	NULL	delta2-36	GP		does not effect					LMP2 RNA	NucleicAcid	levels of			NULL	U3A-701 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_27_20406_s_183	10764778	A mutant of E1A that binds to Stat1 but not to CBP/p300 also down-regulates LMP2 transcription, whereas delta2-36, which binds to neither CBP/p300 nor Stat1, has no effect on the levels of LMP2 RNA in either U3A-701 or 2fTGH cells.	bind
44552	7	11223	5	NULL	NULL	NULL	NULL	delta2-36	GP		does not effect					LMP2 RNA	NucleicAcid	levels of			NULL	2fTGH cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_27_20406_s_183	10764778	A mutant of E1A that binds to Stat1 but not to CBP/p300 also down-regulates LMP2 transcription, whereas delta2-36, which binds to neither CBP/p300 nor Stat1, has no effect on the levels of LMP2 RNA in either U3A-701 or 2fTGH cells.	bind
44553	8	11223	5	NULL	NULL	NULL	NULL	statement 6	Process		is an alternative to					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_27_20406_s_183	10764778	A mutant of E1A that binds to Stat1 but not to CBP/p300 also down-regulates LMP2 transcription, whereas delta2-36, which binds to neither CBP/p300 nor Stat1, has no effect on the levels of LMP2 RNA in either U3A-701 or 2fTGH cells.	bind
44467	1	11223	6	NULL	NULL	0	NULL	E1A	NULL	mutant	bind	NULL				Stat1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20406_s_183	10764778	A mutant of E1A that binds to Stat1 but not to CBP/p300 also down-regulates LMP2 transcription, whereas delta2-36, which binds to neither CBP/p300 nor Stat1, has no effect on the levels of LMP2 RNA in either U3A-701 or 2fTGH cells.	bind
44468	2	11223	6	NULL	NULL	0	NULL	E1A	NULL	mutant	does not bind	NULL				CBP/p300	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20406_s_183	10764778	A mutant of E1A that binds to Stat1 but not to CBP/p300 also down-regulates LMP2 transcription, whereas delta2-36, which binds to neither CBP/p300 nor Stat1, has no effect on the levels of LMP2 RNA in either U3A-701 or 2fTGH cells.	bind
44469	3	11223	6	NULL	NULL	0	NULL	E1A	NULL	mutant	downregulates	NULL				LMP2	NULL	transcription of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20406_s_183	10764778	A mutant of E1A that binds to Stat1 but not to CBP/p300 also down-regulates LMP2 transcription, whereas delta2-36, which binds to neither CBP/p300 nor Stat1, has no effect on the levels of LMP2 RNA in either U3A-701 or 2fTGH cells.	bind
45016	4	11223	6	NULL	NULL	0	NULL	delta2-36	NULL		does not bind	NULL				CBP/p300	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20406_s_183	10764778	A mutant of E1A that binds to Stat1 but not to CBP/p300 also down-regulates LMP2 transcription, whereas delta2-36, which binds to neither CBP/p300 nor Stat1, has no effect on the levels of LMP2 RNA in either U3A-701 or 2fTGH cells.	bind
45017	5	11223	6	NULL	NULL	0	NULL	delta2-36	NULL		does not bind	NULL				Stat1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20406_s_183	10764778	A mutant of E1A that binds to Stat1 but not to CBP/p300 also down-regulates LMP2 transcription, whereas delta2-36, which binds to neither CBP/p300 nor Stat1, has no effect on the levels of LMP2 RNA in either U3A-701 or 2fTGH cells.	bind
45018	6	11223	6	NULL	NULL	0	NULL	delta2-36	NULL		has no effect on	NULL				LMP2 RNA	NULL				NULL	U3A-701 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_27_20406_s_183	10764778	A mutant of E1A that binds to Stat1 but not to CBP/p300 also down-regulates LMP2 transcription, whereas delta2-36, which binds to neither CBP/p300 nor Stat1, has no effect on the levels of LMP2 RNA in either U3A-701 or 2fTGH cells.	bind
45019	7	11223	6	NULL	NULL	0	NULL	delta2-36	NULL		has no effect on	NULL				LMP2 RNA	NULL				NULL	2fTGH cells	0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20406_s_183	10764778	A mutant of E1A that binds to Stat1 but not to CBP/p300 also down-regulates LMP2 transcription, whereas delta2-36, which binds to neither CBP/p300 nor Stat1, has no effect on the levels of LMP2 RNA in either U3A-701 or 2fTGH cells.	bind
51209	8	11223	6	10	NULL	0	NULL	statement 6	NULL		is an alternative to	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20406_s_183	10764778	A mutant of E1A that binds to Stat1 but not to CBP/p300 also down-regulates LMP2 transcription, whereas delta2-36, which binds to neither CBP/p300 nor Stat1, has no effect on the levels of LMP2 RNA in either U3A-701 or 2fTGH cells.	bind
44554	1	11224	5	NULL	NULL	NULL	NULL	Skp2	GP	mutant	does not bind					Cul1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_20_5362_s_30	11032804	A mutant of Skp2 that fails to bind Cul1 is defective in these activities, suggesting that these activities of Skp2 represent SCF functions.	bind
45020	1	11224	6	NULL	NULL	0	NULL	Skp2	NULL	mutant	does not bind	NULL				Cul1	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_19_20_5362_s_30	11032804	A mutant of Skp2 that fails to bind Cul1 is defective in these activities, suggesting that these activities of Skp2 represent SCF functions.	bind
44557	1	11225	5	NULL	NULL	NULL	NULL	p47 phox	GP	mutant	does not bind			W193R;; N-terminal SH3 domain		p22 phox	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_24_23328_s_19	15824103	A mutant p47 phox carrying the W193R substitution in the N-terminal SH3 domain neither binds to p22 phox nor activates gp91 phox ( ,  ), and the substitution of Gln for Pro-156 in the PRR of p22 phox (P156Q), a mutation found in a patient with CGD ( ,  ), leads to a defective binding to p47 phox ( ,  ).	bind
44559	3	11225	5	NULL	NULL	NULL	NULL	p22 phox	GP	mutant	is found in			P156Q;; PRR 		CGD patients	GroupOfPeople				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_24_23328_s_19	15824103	A mutant p47 phox carrying the W193R substitution in the N-terminal SH3 domain neither binds to p22 phox nor activates gp91 phox ( ,  ), and the substitution of Gln for Pro-156 in the PRR of p22 phox (P156Q), a mutation found in a patient with CGD ( ,  ), leads to a defective binding to p47 phox ( ,  ).	bind
44560	4	11225	5	NULL	NULL	NULL	NULL	p22 phox	GP	mutant	does not bind			P156Q;; PRR		p47 phox	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_24_23328_s_19	15824103	A mutant p47 phox carrying the W193R substitution in the N-terminal SH3 domain neither binds to p22 phox nor activates gp91 phox ( ,  ), and the substitution of Gln for Pro-156 in the PRR of p22 phox (P156Q), a mutation found in a patient with CGD ( ,  ), leads to a defective binding to p47 phox ( ,  ).	bind
44589	2	11225	5	NULL	NULL	NULL	NULL	p47 phox	GP	mutant	does not activate			W193R;; N-terminal SH3 domain		gp91 phox	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_24_23328_s_19	15824103	A mutant p47 phox carrying the W193R substitution in the N-terminal SH3 domain neither binds to p22 phox nor activates gp91 phox ( ,  ), and the substitution of Gln for Pro-156 in the PRR of p22 phox (P156Q), a mutation found in a patient with CGD ( ,  ), leads to a defective binding to p47 phox ( ,  ).	bind
45021	1	11225	6	NULL	NULL	0	NULL	p47 phox	NULL	mutant	does not bind	NULL		W193R;; N-terminal SH3 domain		p22 phox	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_24_23328_s_19	15824103	A mutant p47 phox carrying the W193R substitution in the N-terminal SH3 domain neither binds to p22 phox nor activates gp91 phox ( ,  ), and the substitution of Gln for Pro-156 in the PRR of p22 phox (P156Q), a mutation found in a patient with CGD ( ,  ), leads to a defective binding to p47 phox ( ,  ).	bind
45022	2	11225	6	NULL	NULL	0	NULL	p47 phox	NULL	mutant	does not activate	NULL		W193R;; N-terminal SH3 domain		gp91 phox	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_24_23328_s_19	15824103	A mutant p47 phox carrying the W193R substitution in the N-terminal SH3 domain neither binds to p22 phox nor activates gp91 phox ( ,  ), and the substitution of Gln for Pro-156 in the PRR of p22 phox (P156Q), a mutation found in a patient with CGD ( ,  ), leads to a defective binding to p47 phox ( ,  ).	bind
45023	3	11225	6	10	NULL	0	NULL	p22 phox	NULL	mutant	is found in	NULL		P156Q;; PRR 		CGD patients	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_24_23328_s_19	15824103	A mutant p47 phox carrying the W193R substitution in the N-terminal SH3 domain neither binds to p22 phox nor activates gp91 phox ( ,  ), and the substitution of Gln for Pro-156 in the PRR of p22 phox (P156Q), a mutation found in a patient with CGD ( ,  ), leads to a defective binding to p47 phox ( ,  ).	bind
45024	4	11225	6	10	NULL	0	NULL	p22 phox	NULL	mutant	does not bind	NULL		P156Q;; PRR 		p47 phox	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_24_23328_s_19	15824103	A mutant p47 phox carrying the W193R substitution in the N-terminal SH3 domain neither binds to p22 phox nor activates gp91 phox ( ,  ), and the substitution of Gln for Pro-156 in the PRR of p22 phox (P156Q), a mutation found in a patient with CGD ( ,  ), leads to a defective binding to p47 phox ( ,  ).	bind
44591	1	11226	5	NULL	NULL	NULL	NULL	p53	GP	mutant	discriminates between					p53-responsive genes	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_2_321_s_399	11057904	A mutant p53 that discriminates between p53-responsive genes cannot induce apoptosis.	bind
44592	2	11226	5	NULL	NULL	NULL	NULL	statement 1	Process		does not induce					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_2_321_s_399	11057904	A mutant p53 that discriminates between p53-responsive genes cannot induce apoptosis.	bind
45025	1	11226	6	NULL	NULL	0	NULL	p53	NULL	mutant	does not induce	NULL				apoptosis	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_103_2_321_s_399	11057904	A mutant p53 that discriminates between p53-responsive genes cannot induce apoptosis.	bind
45026	2	11226	6	NULL	NULL	0	NULL	p53	NULL	mutant	discriminates between	NULL				p53-responsive genes	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_103_2_321_s_399	11057904	A mutant p53 that discriminates between p53-responsive genes cannot induce apoptosis.	bind
44593	1	11227	5	NULL	NULL	NULL	NULL	PCNA oligonucleotide	NucleicAcid	mutant	does not bind					p53	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_12_s_178	9858527	A mutant PCNA oligonucleotide that we showed previously does not bind p53 ( 70) did not compete effectively for binding with the wild-type PCNA probe (lanes 9 and 10).	bind
44636	2	11227	5	NULL	NULL	NULL	NULL	PCNA oligonucleotide	NucleicAcid	mutant	does not compete for		effectively			PCNA probe	NucleicAcid	binding with;;wild-type			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_12_s_178	9858527	A mutant PCNA oligonucleotide that we showed previously does not bind p53 ( 70) did not compete effectively for binding with the wild-type PCNA probe (lanes 9 and 10).	bind
45027	1	11227	6	NULL	NULL	0	NULL	PCNA oligonucleotide	NULL	mutant	does not bind	NULL				p53	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_1_12_s_178	9858527	A mutant PCNA oligonucleotide that we showed previously does not bind p53 ( 70) did not compete effectively for binding with the wild-type PCNA probe (lanes 9 and 10).	bind
51222	2	11227	6	10	NULL	0	NULL	PCNA oligonucleotide	NULL	mutant	does not compete with	NULL	effectively			PCNA probe	NULL	wild-type;;binding of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_12_s_178	9858527	A mutant PCNA oligonucleotide that we showed previously does not bind p53 ( 70) did not compete effectively for binding with the wild-type PCNA probe (lanes 9 and 10).	bind
44594	1	11228	5	NULL	NULL	NULL	NULL	p47(phox) peptide	AminoAcid	mutant	bind			319-337;;Ser328Glu		filamentous actin	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_febs-lett_580_1_16375898_s_8	16375898	A mutant peptide p47(phox)  (319-337, Ser328Glu) bound to filamentous actin more tightly than to monomer  actin.	bind
44595	2	11228	5	NULL	NULL	NULL	NULL	p47(phox) peptide	AminoAcid	mutant	bind			319-337;;Ser328Glu		monomer actin	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_febs-lett_580_1_16375898_s_8	16375898	A mutant peptide p47(phox)  (319-337, Ser328Glu) bound to filamentous actin more tightly than to monomer  actin.	bind
44596	3	11228	5	NULL	NULL	NULL	NULL	statement 1	Process		more tightly than					statement 2	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_febs-lett_580_1_16375898_s_8	16375898	A mutant peptide p47(phox)  (319-337, Ser328Glu) bound to filamentous actin more tightly than to monomer  actin.	bind
45028	1	11228	6	10	NULL	0	NULL	p47(phox) 	NULL	mutant	bind	NULL		Ser328Glu		filamentous actin	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_febs-lett_580_1_16375898_s_8	16375898	A mutant peptide p47(phox)  (319-337, Ser328Glu) bound to filamentous actin more tightly than to monomer  actin.	bind
45029	2	11228	6	10	NULL	0	NULL	p47(phox)	NULL	mutant	bind	NULL		Ser328Glu		monomer actin	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0570-0579_febs-lett_580_1_16375898_s_8	16375898	A mutant peptide p47(phox)  (319-337, Ser328Glu) bound to filamentous actin more tightly than to monomer  actin.	bind
45030	3	11228	6	NULL	NULL	0	NULL	statement 1	NULL		is higher than	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	abs-batch0570-0579_febs-lett_580_1_16375898_s_8	16375898	A mutant peptide p47(phox)  (319-337, Ser328Glu) bound to filamentous actin more tightly than to monomer  actin.	bind
44597	1	11230	5	NULL	NULL	NULL	NULL	NF- B DNA probe	NucleicAcid	mutant	does not bind					myotrophin	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1589_3_247_s_253	12031792	A mutant probe of NF- B DNA also did not show any binding to myotrophin.	bind
45031	1	11230	6	10	NULL	0	NULL	NF-B DNA probe		mutant	does not bind					myotrophin					NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1589_3_247_s_253	12031792	A mutant probe of NF- B DNA also did not show any binding to myotrophin.	bind
44603	1	11232	5	NULL	NULL	NULL	NULL	RNF4	GP	mutant	does not bind					PATZ	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_5_3280_s_7	11719514	A mutant RNF4 that does not bind PATZ but enhances AR-dependent transcription is not influenced by PATZ, demonstrating that the repression by PATZ occurs only upon binding to RNF4.	bind
44604	2	11232	5	NULL	NULL	NULL	NULL	RNF4	GP	mutant	enhance					transcription	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_5_3280_s_7	11719514	A mutant RNF4 that does not bind PATZ but enhances AR-dependent transcription is not influenced by PATZ, demonstrating that the repression by PATZ occurs only upon binding to RNF4.	bind
44605	3	11232	5	NULL	NULL	NULL	NULL	transcription	Process		is dependent on					AR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_5_3280_s_7	11719514	A mutant RNF4 that does not bind PATZ but enhances AR-dependent transcription is not influenced by PATZ, demonstrating that the repression by PATZ occurs only upon binding to RNF4.	bind
44606	4	11232	5	NULL	NULL	NULL	NULL	statement 2	Process		is not influenced by					PATZ	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_5_3280_s_7	11719514	A mutant RNF4 that does not bind PATZ but enhances AR-dependent transcription is not influenced by PATZ, demonstrating that the repression by PATZ occurs only upon binding to RNF4.	bind
44607	5	11232	5	NULL	NULL	NULL	NULL	PATZ	GP		repress					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_5_3280_s_7	11719514	A mutant RNF4 that does not bind PATZ but enhances AR-dependent transcription is not influenced by PATZ, demonstrating that the repression by PATZ occurs only upon binding to RNF4.	bind
44608	6	11232	5	NULL	NULL	NULL	NULL	PATZ	GP		bind					RNF4	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_5_3280_s_7	11719514	A mutant RNF4 that does not bind PATZ but enhances AR-dependent transcription is not influenced by PATZ, demonstrating that the repression by PATZ occurs only upon binding to RNF4.	bind
44609	7	11232	5	NULL	NULL	NULL	NULL	statement 6	Process		leads to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_5_3280_s_7	11719514	A mutant RNF4 that does not bind PATZ but enhances AR-dependent transcription is not influenced by PATZ, demonstrating that the repression by PATZ occurs only upon binding to RNF4.	bind
45033	1	11232	6	NULL	NULL	0	NULL	RNF4	NULL	mutant	does not bind	NULL				PATZ	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_5_3280_s_7	11719514	A mutant RNF4 that does not bind PATZ but enhances AR-dependent transcription is not influenced by PATZ, demonstrating that the repression by PATZ occurs only upon binding to RNF4.	bind
45034	4	11232	6	NULL	NULL	0	NULL	RNF4	NULL	mutant	enhances	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_5_3280_s_7	11719514	A mutant RNF4 that does not bind PATZ but enhances AR-dependent transcription is not influenced by PATZ, demonstrating that the repression by PATZ occurs only upon binding to RNF4.	bind
52938	3	11232	6	10	NULL	0	NULL	statement 2	NULL		is not influenced by	NULL				PATZ	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_5_3280_s_7	11719514	A mutant RNF4 that does not bind PATZ but enhances AR-dependent transcription is not influenced by PATZ, demonstrating that the repression by PATZ occurs only upon binding to RNF4.	bind
52958	2	11232	6	NULL	NULL	0	NULL	transcription	NULL		is dependent on	NULL				AR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_5_3280_s_7	11719514	A mutant RNF4 that does not bind PATZ but enhances AR-dependent transcription is not influenced by PATZ, demonstrating that the repression by PATZ occurs only upon binding to RNF4.	bind
52959	5	11232	6	NULL	NULL	0	NULL	PATZ	NULL		bind	NULL				RNF4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_5_3280_s_7	11719514	A mutant RNF4 that does not bind PATZ but enhances AR-dependent transcription is not influenced by PATZ, demonstrating that the repression by PATZ occurs only upon binding to RNF4.	bind
52960	6	11232	6	NULL	NULL	0	NULL	PATZ	NULL		represses	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_5_3280_s_7	11719514	A mutant RNF4 that does not bind PATZ but enhances AR-dependent transcription is not influenced by PATZ, demonstrating that the repression by PATZ occurs only upon binding to RNF4.	bind
52961	7	11232	6	NULL	NULL	0	NULL	statement 6	NULL		occurs upon	NULL	only			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_5_3280_s_7	11719514	A mutant RNF4 that does not bind PATZ but enhances AR-dependent transcription is not influenced by PATZ, demonstrating that the repression by PATZ occurs only upon binding to RNF4.	bind
44610	1	11233	5	NULL	NULL	NULL	NULL	Ski protein	GP	mutant	retains					Smad4	GP	binding of	deltaS2/3		NULL		NULL	NULL	NULL	NULL	gw60_cell_111_3_357_s_152	12419246	A mutant Ski protein that retains binding to either Smad4 (deltaS2/3) or Smad2 (W274E) is able to repress activin signaling.	bind
44611	2	11233	5	NULL	NULL	NULL	NULL	Ski protein	GP	mutant	retains					Smad2	GP	binding of	W274E		NULL		NULL	NULL	NULL	NULL	gw60_cell_111_3_357_s_152	12419246	A mutant Ski protein that retains binding to either Smad4 (deltaS2/3) or Smad2 (W274E) is able to repress activin signaling.	bind
44612	3	11233	5	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_111_3_357_s_152	12419246	A mutant Ski protein that retains binding to either Smad4 (deltaS2/3) or Smad2 (W274E) is able to repress activin signaling.	bind
44613	4	11233	5	NULL	NULL	NULL	NULL	statement 1	Process		repress					activin	GP	signaling of			NULL		NULL	NULL	NULL	NULL	gw60_cell_111_3_357_s_152	12419246	A mutant Ski protein that retains binding to either Smad4 (deltaS2/3) or Smad2 (W274E) is able to repress activin signaling.	bind
44614	5	11233	5	NULL	NULL	NULL	NULL	statement 2	Process		repress					activin	GP	signaling of			NULL		NULL	NULL	NULL	NULL	gw60_cell_111_3_357_s_152	12419246	A mutant Ski protein that retains binding to either Smad4 (deltaS2/3) or Smad2 (W274E) is able to repress activin signaling.	bind
45035	1	11233	6	NULL	NULL	0	NULL	Ski protein	NULL	mutant	bind	NULL				Smad4	NULL		deltaS2/3		NULL		0	NULL	NULL	NULL	gw60_cell_111_3_357_s_152	12419246	A mutant Ski protein that retains binding to either Smad4 (deltaS2/3) or Smad2 (W274E) is able to repress activin signaling.	bind
45036	2	11233	6	NULL	NULL	0	NULL	Ski protein	NULL	mutant	bind	NULL				Smad2	NULL		W274E		NULL		0	NULL	NULL	NULL	gw60_cell_111_3_357_s_152	12419246	A mutant Ski protein that retains binding to either Smad4 (deltaS2/3) or Smad2 (W274E) is able to repress activin signaling.	bind
45037	3	11233	6	10	NULL	0	NULL	statement 1	NULL		repress	NULL				activin	NULL	signaling of			NULL		NULL	NULL	NULL	NULL	gw60_cell_111_3_357_s_152	12419246	A mutant Ski protein that retains binding to either Smad4 (deltaS2/3) or Smad2 (W274E) is able to repress activin signaling.	bind
51223	4	11233	6	10	NULL	0	NULL	statement 2	NULL		repress	NULL				activin	NULL	signaling of			NULL		0	NULL	NULL	NULL	gw60_cell_111_3_357_s_152	12419246	A mutant Ski protein that retains binding to either Smad4 (deltaS2/3) or Smad2 (W274E) is able to repress activin signaling.	bind
51224	5	11233	6	10	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_111_3_357_s_152	12419246	A mutant Ski protein that retains binding to either Smad4 (deltaS2/3) or Smad2 (W274E) is able to repress activin signaling.	bind
44851	1	11234	5	NULL	NULL	NULL	NULL	SR-BIdel509	GP		is a mutant of					SR-BI	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_37_34042_s_5	12119305	A mutant SR-BI (SR-BIdel509) that lacked only the leucine in the PDZ-interacting domain failed to interact with PDZK1  in vitro, while showing normal selective uptake function in nonpolarized cells.	bind
44852	2	11234	5	NULL	NULL	NULL	NULL	SR-BIdel509	GP		lacks					SR-BI	GP		leucine;;PDZ-interacting domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_37_34042_s_5	12119305	A mutant SR-BI (SR-BIdel509) that lacked only the leucine in the PDZ-interacting domain failed to interact with PDZK1  in vitro, while showing normal selective uptake function in nonpolarized cells.	bind
44853	3	11234	5	NULL	NULL	NULL	NULL	statement 2	Process		does not interact with					PDZK1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_37_34042_s_5	12119305	A mutant SR-BI (SR-BIdel509) that lacked only the leucine in the PDZ-interacting domain failed to interact with PDZK1  in vitro, while showing normal selective uptake function in nonpolarized cells.	bind
44854	4	11234	5	NULL	NULL	NULL	NULL	statement 2	Process		shows					selective uptake function	Process	normal			NULL	nonpolarized cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_37_34042_s_5	12119305	A mutant SR-BI (SR-BIdel509) that lacked only the leucine in the PDZ-interacting domain failed to interact with PDZK1  in vitro, while showing normal selective uptake function in nonpolarized cells.	bind
45038	1	11234	6	10	NULL	0	NULL	SR-BI		mutant;; lacking	does not interact with			leucine;; PDZ-interacting domain		PDZK1					NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_37_34042_s_5	12119305	A mutant SR-BI (SR-BIdel509) that lacked only the leucine in the PDZ-interacting domain failed to interact with PDZK1  in vitro, while showing normal selective uptake function in nonpolarized cells.	bind
45039	2	11234	6	NULL	NULL	0	NULL	SR-BI	NULL	mutant;; lacking	displays	NULL		leucine;; PDZ-interacting domain		selective uptake	NULL				NULL	nonpolarized cells	0	NULL	NULL	NULL	gw60_jbiolchem_277_37_34042_s_5	12119305	A mutant SR-BI (SR-BIdel509) that lacked only the leucine in the PDZ-interacting domain failed to interact with PDZK1  in vitro, while showing normal selective uptake function in nonpolarized cells.	bind
44856	1	11235	5	NULL	NULL	NULL	NULL	ArpA	GP	mutant	does not bind					DNA target	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_2_326_s_370	15944459	A mutant strain deficient in ArpA or producing a mutant ArpA protein unable to bind to its target DNA overproduces streptomycin and forms aerial mycelia and spores earlier than the wild-type strain ( ,  ).	bind
44857	2	11235	5	NULL	NULL	NULL	NULL	ArpA	GP	mutant	overproduces					streptomycin	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_2_326_s_370	15944459	A mutant strain deficient in ArpA or producing a mutant ArpA protein unable to bind to its target DNA overproduces streptomycin and forms aerial mycelia and spores earlier than the wild-type strain ( ,  ).	bind
44858	3	11235	5	NULL	NULL	NULL	NULL	ArpA	GP	mutant	forms					aerial mycelia	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_2_326_s_370	15944459	A mutant strain deficient in ArpA or producing a mutant ArpA protein unable to bind to its target DNA overproduces streptomycin and forms aerial mycelia and spores earlier than the wild-type strain ( ,  ).	bind
44859	4	11235	5	NULL	NULL	NULL	NULL	ArpA	GP	mutant	forms					spores	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_2_326_s_370	15944459	A mutant strain deficient in ArpA or producing a mutant ArpA protein unable to bind to its target DNA overproduces streptomycin and forms aerial mycelia and spores earlier than the wild-type strain ( ,  ).	bind
44861	5	11235	5	NULL	NULL	NULL	NULL	ArpA	GP	wild-type	forms					aerial mycelia	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_2_326_s_370	15944459	A mutant strain deficient in ArpA or producing a mutant ArpA protein unable to bind to its target DNA overproduces streptomycin and forms aerial mycelia and spores earlier than the wild-type strain ( ,  ).	bind
44862	6	11235	5	NULL	NULL	NULL	NULL	ArpA	GP	wild-type	forms					spores	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_2_326_s_370	15944459	A mutant strain deficient in ArpA or producing a mutant ArpA protein unable to bind to its target DNA overproduces streptomycin and forms aerial mycelia and spores earlier than the wild-type strain ( ,  ).	bind
44863	7	11235	5	NULL	NULL	NULL	NULL	statement 3	Process		occurs earlier than					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_2_326_s_370	15944459	A mutant strain deficient in ArpA or producing a mutant ArpA protein unable to bind to its target DNA overproduces streptomycin and forms aerial mycelia and spores earlier than the wild-type strain ( ,  ).	bind
44864	8	11235	5	NULL	NULL	NULL	NULL	statement 4	Process		occurs earlier than					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_2_326_s_370	15944459	A mutant strain deficient in ArpA or producing a mutant ArpA protein unable to bind to its target DNA overproduces streptomycin and forms aerial mycelia and spores earlier than the wild-type strain ( ,  ).	bind
45040	1	11235	6	NULL	NULL	0	NULL	ArpA	NULL	mutant	does not bind	NULL				target DNA	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_2_326_s_370	15944459	A mutant strain deficient in ArpA or producing a mutant ArpA protein unable to bind to its target DNA overproduces streptomycin and forms aerial mycelia and spores earlier than the wild-type strain ( ,  ).	bind
45041	2	11235	6	NULL	NULL	0	NULL	ArpA	NULL	mutant	overproduces	NULL				streptomycin	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_2_326_s_370	15944459	A mutant strain deficient in ArpA or producing a mutant ArpA protein unable to bind to its target DNA overproduces streptomycin and forms aerial mycelia and spores earlier than the wild-type strain ( ,  ).	bind
45042	3	11235	6	NULL	NULL	0	NULL	ArpA	NULL	mutant	forms	NULL				aerial mycelia	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_2_326_s_370	15944459	A mutant strain deficient in ArpA or producing a mutant ArpA protein unable to bind to its target DNA overproduces streptomycin and forms aerial mycelia and spores earlier than the wild-type strain ( ,  ).	bind
45043	4	11235	6	NULL	NULL	0	NULL	ArpA	NULL	wild type	forms	NULL				aerial mycelia	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_2_326_s_370	15944459	A mutant strain deficient in ArpA or producing a mutant ArpA protein unable to bind to its target DNA overproduces streptomycin and forms aerial mycelia and spores earlier than the wild-type strain ( ,  ).	bind
45044	5	11235	6	NULL	NULL	0	NULL	statement 3	NULL		is earlier than	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_2_326_s_370	15944459	A mutant strain deficient in ArpA or producing a mutant ArpA protein unable to bind to its target DNA overproduces streptomycin and forms aerial mycelia and spores earlier than the wild-type strain ( ,  ).	bind
45045	6	11235	6	NULL	NULL	0	NULL	ArpA	NULL	mutant	forms	NULL				spores	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_2_326_s_370	15944459	A mutant strain deficient in ArpA or producing a mutant ArpA protein unable to bind to its target DNA overproduces streptomycin and forms aerial mycelia and spores earlier than the wild-type strain ( ,  ).	bind
45046	7	11235	6	NULL	NULL	0	NULL	ArpA	NULL	wild type	forms	NULL				spores	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_2_326_s_370	15944459	A mutant strain deficient in ArpA or producing a mutant ArpA protein unable to bind to its target DNA overproduces streptomycin and forms aerial mycelia and spores earlier than the wild-type strain ( ,  ).	bind
45047	8	11235	6	NULL	NULL	0	NULL	statement 6	NULL		is earlier than	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_2_326_s_370	15944459	A mutant strain deficient in ArpA or producing a mutant ArpA protein unable to bind to its target DNA overproduces streptomycin and forms aerial mycelia and spores earlier than the wild-type strain ( ,  ).	bind
44870	1	11236	5	NULL	NULL	NULL	NULL	Tpr-Met protein	GP	mutant	does not bind			Tyr489 Phe		Grb2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_28_19649_s_190	10391903	A mutant Tpr-Met protein (Tyr489  Phe) that fails to bind to Grb2 has significantly impaired transforming activity.	bind
44871	2	11236	5	NULL	NULL	NULL	NULL	statement 1	Process		has impaired					transforming activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_28_19649_s_190	10391903	A mutant Tpr-Met protein (Tyr489  Phe) that fails to bind to Grb2 has significantly impaired transforming activity.	bind
45048	1	11236	6	NULL	NULL	0	NULL	Tpr-Met protein	NULL	mutant	does not bind	NULL				Grb2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_28_19649_s_190	10391903	A mutant Tpr-Met protein (Tyr489  Phe) that fails to bind to Grb2 has significantly impaired transforming activity.	bind
45053	2	11236	6	NULL	NULL	0	NULL	Tpr-Met protein	NULL	mutant	has impaired	NULL				transforming activity	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_28_19649_s_190	10391903	A mutant Tpr-Met protein (Tyr489  Phe) that fails to bind to Grb2 has significantly impaired transforming activity.	bind
44872	1	11237	5	NULL	NULL	NULL	NULL	Tpr-Met protein	GP	mutant	does not bind		selectively			Grb2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_20167_s_5	9242692	A mutant Tpr-Met protein that selectively fails to bind Grb2 has reduced transforming activity, implicating pathways downstream of Grb2 in Tpr-Met mediated cell transformation.	bind
44873	3	11237	5	NULL	NULL	NULL	NULL	Tpr-Met	GP		mediates					cell transformation	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_20167_s_5	9242692	A mutant Tpr-Met protein that selectively fails to bind Grb2 has reduced transforming activity, implicating pathways downstream of Grb2 in Tpr-Met mediated cell transformation.	bind
44874	3	11237	5	NULL	NULL	NULL	NULL	statement 2	Process		implicates					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_20167_s_5	9242692	A mutant Tpr-Met protein that selectively fails to bind Grb2 has reduced transforming activity, implicating pathways downstream of Grb2 in Tpr-Met mediated cell transformation.	bind
51225	2	11237	5	NULL	NULL	NULL	NULL	statement 1	Process		has reduced					transforming activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_32_20167_s_5	9242692	A mutant Tpr-Met protein that selectively fails to bind Grb2 has reduced transforming activity, implicating pathways downstream of Grb2 in Tpr-Met mediated cell transformation.	bind
45054	1	11237	6	NULL	NULL	0	NULL	Tpr-Met protein	NULL	mutant	does not bind	NULL	selectively			Grb2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_32_20167_s_5	9242692	A mutant Tpr-Met protein that selectively fails to bind Grb2 has reduced transforming activity, implicating pathways downstream of Grb2 in Tpr-Met mediated cell transformation.	bind
45057	2	11237	6	NULL	NULL	0	NULL	Tpr-Met 	NULL		mediates	NULL				cell transformation	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_32_20167_s_5	9242692	A mutant Tpr-Met protein that selectively fails to bind Grb2 has reduced transforming activity, implicating pathways downstream of Grb2 in Tpr-Met mediated cell transformation.	bind
45060	3	11237	6	NULL	NULL	0	NULL	Tpr-Met	NULL	mutant	has reduced	NULL				transforming activity	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_32_20167_s_5	9242692	A mutant Tpr-Met protein that selectively fails to bind Grb2 has reduced transforming activity, implicating pathways downstream of Grb2 in Tpr-Met mediated cell transformation.	bind
45061	4	11237	6	NULL	NULL	0	NULL	statement 3	NULL		implicates	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_32_20167_s_5	9242692	A mutant Tpr-Met protein that selectively fails to bind Grb2 has reduced transforming activity, implicating pathways downstream of Grb2 in Tpr-Met mediated cell transformation.	bind
46370	1	11238	5	NULL	NULL	NULL	NULL	Sp1	GP		bind					PKR	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_6_3244_s_331	16339759	A mutant with a nonfunctional ISRE, however, showed similar activity as the p503(WT) for both Sp1 and Sp3, further establishing that the binding of Sp1 and Sp3 to the  PKR promoter and basal transcriptional activation by these factors are independent of the ISRE. Sp1 has been shown to function as a gene activator by recruiting TFIID ( ), and the TBP-associated factor 1 (TAF1) activates the TATA-less cyclin D1 promoter by interacting with the Sp1 protein ( ).	bind
46371	2	11238	5	NULL	NULL	NULL	NULL	Sp3	GP		bind					PKR	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_6_3244_s_331	16339759	A mutant with a nonfunctional ISRE, however, showed similar activity as the p503(WT) for both Sp1 and Sp3, further establishing that the binding of Sp1 and Sp3 to the  PKR promoter and basal transcriptional activation by these factors are independent of the ISRE. Sp1 has been shown to function as a gene activator by recruiting TFIID ( ), and the TBP-associated factor 1 (TAF1) activates the TATA-less cyclin D1 promoter by interacting with the Sp1 protein ( ).	bind
46372	3	11238	5	NULL	NULL	NULL	NULL	Sp1	GP		activates					PKR	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_6_3244_s_331	16339759	A mutant with a nonfunctional ISRE, however, showed similar activity as the p503(WT) for both Sp1 and Sp3, further establishing that the binding of Sp1 and Sp3 to the  PKR promoter and basal transcriptional activation by these factors are independent of the ISRE. Sp1 has been shown to function as a gene activator by recruiting TFIID ( ), and the TBP-associated factor 1 (TAF1) activates the TATA-less cyclin D1 promoter by interacting with the Sp1 protein ( ).	bind
46373	4	11238	5	NULL	NULL	NULL	NULL	Sp3	GP		activates					PKR	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_6_3244_s_331	16339759	A mutant with a nonfunctional ISRE, however, showed similar activity as the p503(WT) for both Sp1 and Sp3, further establishing that the binding of Sp1 and Sp3 to the  PKR promoter and basal transcriptional activation by these factors are independent of the ISRE. Sp1 has been shown to function as a gene activator by recruiting TFIID ( ), and the TBP-associated factor 1 (TAF1) activates the TATA-less cyclin D1 promoter by interacting with the Sp1 protein ( ).	bind
46374	5	11238	5	NULL	NULL	NULL	NULL	statement 3	Process		is independent of					ISRE	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_6_3244_s_331	16339759	A mutant with a nonfunctional ISRE, however, showed similar activity as the p503(WT) for both Sp1 and Sp3, further establishing that the binding of Sp1 and Sp3 to the  PKR promoter and basal transcriptional activation by these factors are independent of the ISRE. Sp1 has been shown to function as a gene activator by recruiting TFIID ( ), and the TBP-associated factor 1 (TAF1) activates the TATA-less cyclin D1 promoter by interacting with the Sp1 protein ( ).	bind
46375	6	11238	5	NULL	NULL	NULL	NULL	statement 4	Process		is independent of					ISRE	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_6_3244_s_331	16339759	A mutant with a nonfunctional ISRE, however, showed similar activity as the p503(WT) for both Sp1 and Sp3, further establishing that the binding of Sp1 and Sp3 to the  PKR promoter and basal transcriptional activation by these factors are independent of the ISRE. Sp1 has been shown to function as a gene activator by recruiting TFIID ( ), and the TBP-associated factor 1 (TAF1) activates the TATA-less cyclin D1 promoter by interacting with the Sp1 protein ( ).	bind
46376	7	11238	5	NULL	NULL	NULL	NULL	Sp1	GP		recruits					TFIID	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_6_3244_s_331	16339759	A mutant with a nonfunctional ISRE, however, showed similar activity as the p503(WT) for both Sp1 and Sp3, further establishing that the binding of Sp1 and Sp3 to the  PKR promoter and basal transcriptional activation by these factors are independent of the ISRE. Sp1 has been shown to function as a gene activator by recruiting TFIID ( ), and the TBP-associated factor 1 (TAF1) activates the TATA-less cyclin D1 promoter by interacting with the Sp1 protein ( ).	bind
46377	8	11238	5	NULL	NULL	NULL	NULL	Sp1	GP		acts as					gene activator	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_6_3244_s_331	16339759	A mutant with a nonfunctional ISRE, however, showed similar activity as the p503(WT) for both Sp1 and Sp3, further establishing that the binding of Sp1 and Sp3 to the  PKR promoter and basal transcriptional activation by these factors are independent of the ISRE. Sp1 has been shown to function as a gene activator by recruiting TFIID ( ), and the TBP-associated factor 1 (TAF1) activates the TATA-less cyclin D1 promoter by interacting with the Sp1 protein ( ).	bind
46378	9	11238	5	NULL	NULL	NULL	NULL	statement 7	Process		leads to					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_6_3244_s_331	16339759	A mutant with a nonfunctional ISRE, however, showed similar activity as the p503(WT) for both Sp1 and Sp3, further establishing that the binding of Sp1 and Sp3 to the  PKR promoter and basal transcriptional activation by these factors are independent of the ISRE. Sp1 has been shown to function as a gene activator by recruiting TFIID ( ), and the TBP-associated factor 1 (TAF1) activates the TATA-less cyclin D1 promoter by interacting with the Sp1 protein ( ).	bind
46379	10	11238	5	NULL	NULL	NULL	NULL	TAF1	GP		interacts with					Sp1 protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_6_3244_s_331	16339759	A mutant with a nonfunctional ISRE, however, showed similar activity as the p503(WT) for both Sp1 and Sp3, further establishing that the binding of Sp1 and Sp3 to the  PKR promoter and basal transcriptional activation by these factors are independent of the ISRE. Sp1 has been shown to function as a gene activator by recruiting TFIID ( ), and the TBP-associated factor 1 (TAF1) activates the TATA-less cyclin D1 promoter by interacting with the Sp1 protein ( ).	bind
46380	11	11238	5	NULL	NULL	NULL	NULL	TAF1	GP		is					TBP-associated factor 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_6_3244_s_331	16339759	A mutant with a nonfunctional ISRE, however, showed similar activity as the p503(WT) for both Sp1 and Sp3, further establishing that the binding of Sp1 and Sp3 to the  PKR promoter and basal transcriptional activation by these factors are independent of the ISRE. Sp1 has been shown to function as a gene activator by recruiting TFIID ( ), and the TBP-associated factor 1 (TAF1) activates the TATA-less cyclin D1 promoter by interacting with the Sp1 protein ( ).	bind
46381	12	11238	5	NULL	NULL	NULL	NULL	TAF1	GP		activates					cyclin D1	GP			TATA-less promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_6_3244_s_331	16339759	A mutant with a nonfunctional ISRE, however, showed similar activity as the p503(WT) for both Sp1 and Sp3, further establishing that the binding of Sp1 and Sp3 to the  PKR promoter and basal transcriptional activation by these factors are independent of the ISRE. Sp1 has been shown to function as a gene activator by recruiting TFIID ( ), and the TBP-associated factor 1 (TAF1) activates the TATA-less cyclin D1 promoter by interacting with the Sp1 protein ( ).	bind
46382	13	11238	5	NULL	NULL	NULL	NULL	statement 12	Process		depends on					statement 11	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_6_3244_s_331	16339759	A mutant with a nonfunctional ISRE, however, showed similar activity as the p503(WT) for both Sp1 and Sp3, further establishing that the binding of Sp1 and Sp3 to the  PKR promoter and basal transcriptional activation by these factors are independent of the ISRE. Sp1 has been shown to function as a gene activator by recruiting TFIID ( ), and the TBP-associated factor 1 (TAF1) activates the TATA-less cyclin D1 promoter by interacting with the Sp1 protein ( ).	bind
45762	1	11238	6	NULL	NULL	0	NULL	Sp1	NULL		bind	NULL				PKR	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_6_3244_s_331	16339759	A mutant with a nonfunctional ISRE, however, showed similar activity as the p503(WT) for both Sp1 and Sp3, further establishing that the binding of Sp1 and Sp3 to the  PKR promoter and basal transcriptional activation by these factors are independent of the ISRE. Sp1 has been shown to function as a gene activator by recruiting TFIID ( ), and the TBP-associated factor 1 (TAF1) activates the TATA-less cyclin D1 promoter by interacting with the Sp1 protein ( ).	bind
45763	2	11238	6	NULL	NULL	0	NULL	Sp3	NULL		bind	NULL				PKR	NULL			promoter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_6_3244_s_331	16339759	A mutant with a nonfunctional ISRE, however, showed similar activity as the p503(WT) for both Sp1 and Sp3, further establishing that the binding of Sp1 and Sp3 to the  PKR promoter and basal transcriptional activation by these factors are independent of the ISRE. Sp1 has been shown to function as a gene activator by recruiting TFIID ( ), and the TBP-associated factor 1 (TAF1) activates the TATA-less cyclin D1 promoter by interacting with the Sp1 protein ( ).	bind
45764	3	11238	6	NULL	NULL	0	NULL	Sp1	NULL		activates	NULL				PKR	NULL	transcription of 			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_6_3244_s_331	16339759	A mutant with a nonfunctional ISRE, however, showed similar activity as the p503(WT) for both Sp1 and Sp3, further establishing that the binding of Sp1 and Sp3 to the  PKR promoter and basal transcriptional activation by these factors are independent of the ISRE. Sp1 has been shown to function as a gene activator by recruiting TFIID ( ), and the TBP-associated factor 1 (TAF1) activates the TATA-less cyclin D1 promoter by interacting with the Sp1 protein ( ).	bind
45765	4	11238	6	NULL	NULL	0	NULL	Sp3	NULL		activates	NULL				PKR	NULL	transcription of 			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_6_3244_s_331	16339759	A mutant with a nonfunctional ISRE, however, showed similar activity as the p503(WT) for both Sp1 and Sp3, further establishing that the binding of Sp1 and Sp3 to the  PKR promoter and basal transcriptional activation by these factors are independent of the ISRE. Sp1 has been shown to function as a gene activator by recruiting TFIID ( ), and the TBP-associated factor 1 (TAF1) activates the TATA-less cyclin D1 promoter by interacting with the Sp1 protein ( ).	bind
45766	5	11238	6	NULL	NULL	0	NULL	statement 3	NULL		is independent of	NULL					NULL			ISRE	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_6_3244_s_331	16339759	A mutant with a nonfunctional ISRE, however, showed similar activity as the p503(WT) for both Sp1 and Sp3, further establishing that the binding of Sp1 and Sp3 to the  PKR promoter and basal transcriptional activation by these factors are independent of the ISRE. Sp1 has been shown to function as a gene activator by recruiting TFIID ( ), and the TBP-associated factor 1 (TAF1) activates the TATA-less cyclin D1 promoter by interacting with the Sp1 protein ( ).	bind
45767	6	11238	6	NULL	NULL	0	NULL	statement 4	NULL		is independent of	NULL					NULL			ISRE	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_6_3244_s_331	16339759	A mutant with a nonfunctional ISRE, however, showed similar activity as the p503(WT) for both Sp1 and Sp3, further establishing that the binding of Sp1 and Sp3 to the  PKR promoter and basal transcriptional activation by these factors are independent of the ISRE. Sp1 has been shown to function as a gene activator by recruiting TFIID ( ), and the TBP-associated factor 1 (TAF1) activates the TATA-less cyclin D1 promoter by interacting with the Sp1 protein ( ).	bind
45768	7	11238	6	NULL	NULL	0	NULL	Sp1	NULL		recruits	NULL				TFIID	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_6_3244_s_331	16339759	A mutant with a nonfunctional ISRE, however, showed similar activity as the p503(WT) for both Sp1 and Sp3, further establishing that the binding of Sp1 and Sp3 to the  PKR promoter and basal transcriptional activation by these factors are independent of the ISRE. Sp1 has been shown to function as a gene activator by recruiting TFIID ( ), and the TBP-associated factor 1 (TAF1) activates the TATA-less cyclin D1 promoter by interacting with the Sp1 protein ( ).	bind
45769	8	11238	6	NULL	NULL	0	NULL	Sp1	NULL		acts as a 	NULL				gene activator	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_6_3244_s_331	16339759	A mutant with a nonfunctional ISRE, however, showed similar activity as the p503(WT) for both Sp1 and Sp3, further establishing that the binding of Sp1 and Sp3 to the  PKR promoter and basal transcriptional activation by these factors are independent of the ISRE. Sp1 has been shown to function as a gene activator by recruiting TFIID ( ), and the TBP-associated factor 1 (TAF1) activates the TATA-less cyclin D1 promoter by interacting with the Sp1 protein ( ).	bind
45770	9	11238	6	NULL	NULL	0	NULL	statement 8	NULL		is because of	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_6_3244_s_331	16339759	A mutant with a nonfunctional ISRE, however, showed similar activity as the p503(WT) for both Sp1 and Sp3, further establishing that the binding of Sp1 and Sp3 to the  PKR promoter and basal transcriptional activation by these factors are independent of the ISRE. Sp1 has been shown to function as a gene activator by recruiting TFIID ( ), and the TBP-associated factor 1 (TAF1) activates the TATA-less cyclin D1 promoter by interacting with the Sp1 protein ( ).	bind
45771	10	11238	6	NULL	NULL	0	NULL	TAF1	NULL		is	NULL				TBP-associated factor1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_6_3244_s_331	16339759	A mutant with a nonfunctional ISRE, however, showed similar activity as the p503(WT) for both Sp1 and Sp3, further establishing that the binding of Sp1 and Sp3 to the  PKR promoter and basal transcriptional activation by these factors are independent of the ISRE. Sp1 has been shown to function as a gene activator by recruiting TFIID ( ), and the TBP-associated factor 1 (TAF1) activates the TATA-less cyclin D1 promoter by interacting with the Sp1 protein ( ).	bind
45772	11	11238	6	NULL	NULL	0	NULL	TAF1	NULL		interacts with	NULL				Sp1 protein	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_6_3244_s_331	16339759	A mutant with a nonfunctional ISRE, however, showed similar activity as the p503(WT) for both Sp1 and Sp3, further establishing that the binding of Sp1 and Sp3 to the  PKR promoter and basal transcriptional activation by these factors are independent of the ISRE. Sp1 has been shown to function as a gene activator by recruiting TFIID ( ), and the TBP-associated factor 1 (TAF1) activates the TATA-less cyclin D1 promoter by interacting with the Sp1 protein ( ).	bind
45773	12	11238	6	10	NULL	0	NULL	TAF1	NULL		activates	NULL				cyclin D1	NULL			TATA-less promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_6_3244_s_331	16339759	A mutant with a nonfunctional ISRE, however, showed similar activity as the p503(WT) for both Sp1 and Sp3, further establishing that the binding of Sp1 and Sp3 to the  PKR promoter and basal transcriptional activation by these factors are independent of the ISRE. Sp1 has been shown to function as a gene activator by recruiting TFIID ( ), and the TBP-associated factor 1 (TAF1) activates the TATA-less cyclin D1 promoter by interacting with the Sp1 protein ( ).	bind
46358	13	11238	6	NULL	NULL	0	NULL	statement 12	NULL		depends on	NULL				statement 11	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_6_3244_s_331	16339759	A mutant with a nonfunctional ISRE, however, showed similar activity as the p503(WT) for both Sp1 and Sp3, further establishing that the binding of Sp1 and Sp3 to the  PKR promoter and basal transcriptional activation by these factors are independent of the ISRE. Sp1 has been shown to function as a gene activator by recruiting TFIID ( ), and the TBP-associated factor 1 (TAF1) activates the TATA-less cyclin D1 promoter by interacting with the Sp1 protein ( ).	bind
44875	1	11239	5	NULL	NULL	NULL	NULL			mutant	does not bind			Y205A		LDL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_11_7018_s_66	10066756	A mutant with alanine at this position (Y205A) did not bind to LDL (Fig.  1).	bind
45063	1	11239	6	10	NULL	0	NULL		NULL	mutant	does not bind	NULL		Y205A		LDL	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_11_7018_s_66	10066756	A mutant with alanine at this position (Y205A) did not bind to LDL (Fig.  1).	bind
44876	1	11240	5	NULL	NULL	NULL	NULL	rIB2	GP		bind					p38	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4073_s_232	12024021	A mutant with the first 306 amino acids deleted, which eliminated rIB2 binding to p38 (rIB2-deltan306), failed to fully promote p38 activation when expressed alone or when coexpressed with Tiam1 (Fig.  7A, upper panel, lanes 5 and 8).	bind
44877	2	11240	5	NULL	NULL	NULL	NULL	rIB2-deltan306	GP		is formed from					rIB2	GP	deletion of	first 306 amino acids		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4073_s_232	12024021	A mutant with the first 306 amino acids deleted, which eliminated rIB2 binding to p38 (rIB2-deltan306), failed to fully promote p38 activation when expressed alone or when coexpressed with Tiam1 (Fig.  7A, upper panel, lanes 5 and 8).	bind
44878	3	11240	5	NULL	NULL	NULL	NULL	rIB2-deltan306	GP		eliminates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4073_s_232	12024021	A mutant with the first 306 amino acids deleted, which eliminated rIB2 binding to p38 (rIB2-deltan306), failed to fully promote p38 activation when expressed alone or when coexpressed with Tiam1 (Fig.  7A, upper panel, lanes 5 and 8).	bind
44879	4	11240	5	NULL	NULL	NULL	NULL	rIB2-deltan306	GP		does not promote		fully			p38	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4073_s_232	12024021	A mutant with the first 306 amino acids deleted, which eliminated rIB2 binding to p38 (rIB2-deltan306), failed to fully promote p38 activation when expressed alone or when coexpressed with Tiam1 (Fig.  7A, upper panel, lanes 5 and 8).	bind
45065	1	11240	6	NULL	NULL	0	NULL	rIB2	NULL		bind	NULL				p38	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_12_4073_s_232	12024021	A mutant with the first 306 amino acids deleted, which eliminated rIB2 binding to p38 (rIB2-deltan306), failed to fully promote p38 activation when expressed alone or when coexpressed with Tiam1 (Fig.  7A, upper panel, lanes 5 and 8).	bind
45070	2	11240	6	NULL	NULL	0	NULL	rIB2	NULL	mutant;;deletion of	failed to promote	NULL		first 306 amino acids		p38	NULL	activation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4073_s_232	12024021	A mutant with the first 306 amino acids deleted, which eliminated rIB2 binding to p38 (rIB2-deltan306), failed to fully promote p38 activation when expressed alone or when coexpressed with Tiam1 (Fig.  7A, upper panel, lanes 5 and 8).	bind
51241	3	11240	6	10	NULL	0	NULL	rIB2-deltan306			is formed from					 rIB2		deletion of	first 306 amino acids		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4073_s_232	12024021	A mutant with the first 306 amino acids deleted, which eliminated rIB2 binding to p38 (rIB2-deltan306), failed to fully promote p38 activation when expressed alone or when coexpressed with Tiam1 (Fig.  7A, upper panel, lanes 5 and 8).	bind
51242	4	11240	6	10	NULL	0	NULL	rIB2-deltan306	NULL		eliminates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_12_4073_s_232	12024021	A mutant with the first 306 amino acids deleted, which eliminated rIB2 binding to p38 (rIB2-deltan306), failed to fully promote p38 activation when expressed alone or when coexpressed with Tiam1 (Fig.  7A, upper panel, lanes 5 and 8).	bind
44885	1	11241	5	NULL	NULL	NULL	NULL	T	GP		bind					p130	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_8_3679_s_118	9108037	A mutant within the putative J-domain helix 3 does not impair T binding to p130, but prevents T-mediated alteration of its phosphorylation state, thus implying that an N-terminal region could influence cell cycle-dependent posttranslational modifications of p130 ( 29).	bind
44886	2	11241	5	NULL	NULL	NULL	NULL			mutant;;putative 	does not impair			J-domain helix 3		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_8_3679_s_118	9108037	A mutant within the putative J-domain helix 3 does not impair T binding to p130, but prevents T-mediated alteration of its phosphorylation state, thus implying that an N-terminal region could influence cell cycle-dependent posttranslational modifications of p130 ( 29).	bind
44887	3	11241	5	NULL	NULL	NULL	NULL	T	GP		mediate					p130	GP	alteration of phosphorylation state			NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_8_3679_s_118	9108037	A mutant within the putative J-domain helix 3 does not impair T binding to p130, but prevents T-mediated alteration of its phosphorylation state, thus implying that an N-terminal region could influence cell cycle-dependent posttranslational modifications of p130 ( 29).	bind
44888	4	11241	5	NULL	NULL	NULL	NULL	statement 2	Process		prevents					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_8_3679_s_118	9108037	A mutant within the putative J-domain helix 3 does not impair T binding to p130, but prevents T-mediated alteration of its phosphorylation state, thus implying that an N-terminal region could influence cell cycle-dependent posttranslational modifications of p130 ( 29).	bind
44889	5	11241	5	NULL	NULL	NULL	NULL	p130	GP	posttranslational modifications of	is dependent on					cell cycle	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_8_3679_s_118	9108037	A mutant within the putative J-domain helix 3 does not impair T binding to p130, but prevents T-mediated alteration of its phosphorylation state, thus implying that an N-terminal region could influence cell cycle-dependent posttranslational modifications of p130 ( 29).	bind
44890	6	11241	5	NULL	NULL	NULL	NULL	T	GP		influences			N-terminal region		statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_8_3679_s_118	9108037	A mutant within the putative J-domain helix 3 does not impair T binding to p130, but prevents T-mediated alteration of its phosphorylation state, thus implying that an N-terminal region could influence cell cycle-dependent posttranslational modifications of p130 ( 29).	bind
45075	1	11241	6	NULL	NULL	0	NULL	T 	NULL		bind	NULL				p130	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_94_8_3679_s_118	9108037	A mutant within the putative J-domain helix 3 does not impair T binding to p130, but prevents T-mediated alteration of its phosphorylation state, thus implying that an N-terminal region could influence cell cycle-dependent posttranslational modifications of p130 ( 29).	bind
45096	2	11241	6	NULL	NULL	0	NULL		NULL	mutant;; putative	does not impair	NULL		J-domain helix 3		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_94_8_3679_s_118	9108037	A mutant within the putative J-domain helix 3 does not impair T binding to p130, but prevents T-mediated alteration of its phosphorylation state, thus implying that an N-terminal region could influence cell cycle-dependent posttranslational modifications of p130 ( 29).	bind
45097	6	11241	6	10	NULL	0	NULL		NULL		influences	NULL		N-terminal region		statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_8_3679_s_118	9108037	A mutant within the putative J-domain helix 3 does not impair T binding to p130, but prevents T-mediated alteration of its phosphorylation state, thus implying that an N-terminal region could influence cell cycle-dependent posttranslational modifications of p130 ( 29).	bind
51243	3	11241	6	10	NULL	0	NULL	T	NULL		mediate	NULL				p130	NULL	alteration of  phosphorylation state			NULL		0	NULL	NULL	NULL	gw60_pnas_94_8_3679_s_118	9108037	A mutant within the putative J-domain helix 3 does not impair T binding to p130, but prevents T-mediated alteration of its phosphorylation state, thus implying that an N-terminal region could influence cell cycle-dependent posttranslational modifications of p130 ( 29).	bind
51244	4	11241	6	10	NULL	0	NULL	statement 2	NULL		prevents	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_94_8_3679_s_118	9108037	A mutant within the putative J-domain helix 3 does not impair T binding to p130, but prevents T-mediated alteration of its phosphorylation state, thus implying that an N-terminal region could influence cell cycle-dependent posttranslational modifications of p130 ( 29).	bind
51245	5	11241	6	10	NULL	NULL	NULL	p130		posttranslational modifications of	depends on					cell cycle					NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_8_3679_s_118	9108037	A mutant within the putative J-domain helix 3 does not impair T binding to p130, but prevents T-mediated alteration of its phosphorylation state, thus implying that an N-terminal region could influence cell cycle-dependent posttranslational modifications of p130 ( 29).	bind
44891	1	11242	5	NULL	NULL	NULL	NULL	RNA polymerase II	GP	mutant;;yeast	lacks								subunit Rpb9		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_26_24189_s_257	12692127	A mutant yeast RNA  polymerase II lacking subunit Rpb9 (RPIIdelta9) is significantly impaired in  its ability to respond to TFIIS-stimulated readthrough of elongation blocks,  although the mutant polymerase binds TFIIS as well as wild type polymerase  ( ).	bind
44892	2	11242	5	NULL	NULL	NULL	NULL	statement 1	Process		is					RPIIdelta9	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_26_24189_s_257	12692127	A mutant yeast RNA  polymerase II lacking subunit Rpb9 (RPIIdelta9) is significantly impaired in  its ability to respond to TFIIS-stimulated readthrough of elongation blocks,  although the mutant polymerase binds TFIIS as well as wild type polymerase  ( ).	bind
44893	3	11242	5	NULL	NULL	NULL	NULL	TFIIS	GP		stimulate					elongation blocks	NucleicAcid	readthrough of 			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_26_24189_s_257	12692127	A mutant yeast RNA  polymerase II lacking subunit Rpb9 (RPIIdelta9) is significantly impaired in  its ability to respond to TFIIS-stimulated readthrough of elongation blocks,  although the mutant polymerase binds TFIIS as well as wild type polymerase  ( ).	bind
44895	4	11242	5	NULL	NULL	NULL	NULL	RPIIdelta9	GP		impairs		significantly			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_26_24189_s_257	12692127	A mutant yeast RNA  polymerase II lacking subunit Rpb9 (RPIIdelta9) is significantly impaired in  its ability to respond to TFIIS-stimulated readthrough of elongation blocks,  although the mutant polymerase binds TFIIS as well as wild type polymerase  ( ).	bind
44896	6	11242	5	NULL	NULL	NULL	NULL	RPIIdelta9	GP		bind					TFIIS	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_26_24189_s_257	12692127	A mutant yeast RNA  polymerase II lacking subunit Rpb9 (RPIIdelta9) is significantly impaired in  its ability to respond to TFIIS-stimulated readthrough of elongation blocks,  although the mutant polymerase binds TFIIS as well as wild type polymerase  ( ).	bind
44897	5	11242	5	NULL	NULL	NULL	NULL	RNA polymerase II	GP	wild type	bind					TFIIS	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_26_24189_s_257	12692127	A mutant yeast RNA  polymerase II lacking subunit Rpb9 (RPIIdelta9) is significantly impaired in  its ability to respond to TFIIS-stimulated readthrough of elongation blocks,  although the mutant polymerase binds TFIIS as well as wild type polymerase  ( ).	bind
45098	1	11242	6	NULL	NULL	0	NULL	RNA polymerase II 	NULL	mutant;; yeast	lacks	NULL					NULL		Rpb9 subunit		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_26_24189_s_257	12692127	A mutant yeast RNA  polymerase II lacking subunit Rpb9 (RPIIdelta9) is significantly impaired in  its ability to respond to TFIIS-stimulated readthrough of elongation blocks,  although the mutant polymerase binds TFIIS as well as wild type polymerase  ( ).	bind
45099	2	11242	6	NULL	NULL	0	NULL	RNA polymerase II	NULL	yeast;; mutant	bind	NULL				TFIIS	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_26_24189_s_257	12692127	A mutant yeast RNA  polymerase II lacking subunit Rpb9 (RPIIdelta9) is significantly impaired in  its ability to respond to TFIIS-stimulated readthrough of elongation blocks,  although the mutant polymerase binds TFIIS as well as wild type polymerase  ( ).	bind
45100	3	11242	6	NULL	NULL	0	NULL	RNA polymerase II	NULL	yeast;; mutant	bind	NULL				polymerase	NULL	wild type			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_26_24189_s_257	12692127	A mutant yeast RNA  polymerase II lacking subunit Rpb9 (RPIIdelta9) is significantly impaired in  its ability to respond to TFIIS-stimulated readthrough of elongation blocks,  although the mutant polymerase binds TFIIS as well as wild type polymerase  ( ).	bind
45101	4	11242	6	NULL	NULL	0	NULL	TFIIS	NULL		stimulates	NULL				elongation blocks	NULL	readthrough of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_26_24189_s_257	12692127	A mutant yeast RNA  polymerase II lacking subunit Rpb9 (RPIIdelta9) is significantly impaired in  its ability to respond to TFIIS-stimulated readthrough of elongation blocks,  although the mutant polymerase binds TFIIS as well as wild type polymerase  ( ).	bind
45102	5	11242	6	NULL	NULL	0	NULL	RNA polymerase II	NULL	mutant;; yeast	impairs	NULL	significantly			statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_26_24189_s_257	12692127	A mutant yeast RNA  polymerase II lacking subunit Rpb9 (RPIIdelta9) is significantly impaired in  its ability to respond to TFIIS-stimulated readthrough of elongation blocks,  although the mutant polymerase binds TFIIS as well as wild type polymerase  ( ).	bind
51246	6	11242	6	10	NULL	0	NULL	RPIIdelta9	NULL		is	NULL				RNA polymerase II	NULL	mutant	lacking subunit Rpb9		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_26_24189_s_257	12692127	A mutant yeast RNA  polymerase II lacking subunit Rpb9 (RPIIdelta9) is significantly impaired in  its ability to respond to TFIIS-stimulated readthrough of elongation blocks,  although the mutant polymerase binds TFIIS as well as wild type polymerase  ( ).	bind
44898	1	11243	5	NULL	NULL	NULL	NULL	bcl-X  oligonucleotide	NucleicAcid	mutant	bind		less efficiently		HRE	PR	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_11_9831_s_216	14679196	A mutated  bcl-X HRE oligonucleotide binds less efficiently to PR.	bind
45103	1	11243	6	NULL	NULL	0	NULL	bcl-X oligonucleotide	NULL	mutant	bind	NULL	less efficiently		HRE	PR	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_11_9831_s_216	14679196	A mutated  bcl-X HRE oligonucleotide binds less efficiently to PR.	bind
44899	1	11244	5	NULL	NULL	NULL	NULL	nuclear proteins	GP		isolated from					HEK 293T cells	Cell	PKD2-transfected			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3423_s_129	10207066	A mutated AP-1 oligonucleotide failed to bind nuclear proteins isolated from PKD2-transfected HEK 293T cells.	bind
44900	2	11244	5	NULL	NULL	NULL	NULL	AP-1 oligonucleotide	NucleicAcid	mutant	does not bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3423_s_129	10207066	A mutated AP-1 oligonucleotide failed to bind nuclear proteins isolated from PKD2-transfected HEK 293T cells.	bind
45104	1	11244	6	NULL	NULL	0	NULL	nuclear proteins	NULL		isolated from	NULL				HEK 293T cells	NULL	PKD2-transfected			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3423_s_129	10207066	A mutated AP-1 oligonucleotide failed to bind nuclear proteins isolated from PKD2-transfected HEK 293T cells.	bind
45105	2	11244	6	NULL	NULL	0	NULL	AP-1 oligonucleotide	NULL	mutant	does not bind	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3423_s_129	10207066	A mutated AP-1 oligonucleotide failed to bind nuclear proteins isolated from PKD2-transfected HEK 293T cells.	bind
44901	1	11245	5	NULL	NULL	NULL	NULL	perlecan	GP	mutant	does not contain			domain I					GAG chains		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_15061_s_124	11847210	A mutated form of perlecan domain I containing no GAG chains did not bind PRELP (Fig.  3 B).	bind
44902	2	11245	5	NULL	NULL	NULL	NULL	statement 1	Process		does not bind					PRELP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_17_15061_s_124	11847210	A mutated form of perlecan domain I containing no GAG chains did not bind PRELP (Fig.  3 B).	bind
45106	1	11245	6	NULL	NULL	0	NULL	perlecan	NULL	mutant	does not contain	NULL		domain I			NULL		GAG chains		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_17_15061_s_124	11847210	A mutated form of perlecan domain I containing no GAG chains did not bind PRELP (Fig.  3 B).	bind
45107	2	11245	6	NULL	NULL	0	NULL	statement 1	NULL		does not bind	NULL				PRELP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_17_15061_s_124	11847210	A mutated form of perlecan domain I containing no GAG chains did not bind PRELP (Fig.  3 B).	bind
44903	1	11246	5	NULL	NULL	NULL	NULL	statement 1	Process		does not bind					JNK	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5383_1671_s_95	9733513	A mutated JIP-1 molecule with an in-frame deletion of the JNK binding domain did not bind JNK but did bind MKK7, DLK, MLK3, and HPK1 ( Fig. 3A).	bind
44904	3	11246	5	NULL	NULL	NULL	NULL	statement 1	Process		bind					MKK7	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5383_1671_s_95	9733513	A mutated JIP-1 molecule with an in-frame deletion of the JNK binding domain did not bind JNK but did bind MKK7, DLK, MLK3, and HPK1 ( Fig. 3A).	bind
44905	4	11246	5	NULL	NULL	NULL	NULL	statement 1	Process		bind					DLK	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5383_1671_s_95	9733513	A mutated JIP-1 molecule with an in-frame deletion of the JNK binding domain did not bind JNK but did bind MKK7, DLK, MLK3, and HPK1 ( Fig. 3A).	bind
44906	5	11246	5	NULL	NULL	NULL	NULL	statement 1	Process		bind					MLK3	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5383_1671_s_95	9733513	A mutated JIP-1 molecule with an in-frame deletion of the JNK binding domain did not bind JNK but did bind MKK7, DLK, MLK3, and HPK1 ( Fig. 3A).	bind
44907	6	11246	5	NULL	NULL	NULL	NULL	statement 1	Process		bind					HPK1	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5383_1671_s_95	9733513	A mutated JIP-1 molecule with an in-frame deletion of the JNK binding domain did not bind JNK but did bind MKK7, DLK, MLK3, and HPK1 ( Fig. 3A).	bind
68149	1	11246	5	NULL	NULL	NULL	NULL	JIP-1	GP	deletion mutant	lacks					JNK binding domain	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5383_1671_s_95	9733513	A mutated JIP-1 molecule with an in-frame deletion of the JNK binding domain did not bind JNK but did bind MKK7, DLK, MLK3, and HPK1 ( Fig. 3A).	bind
45108	1	11246	6	10	NULL	0	NULL	JIP-1 molecule	NULL	deletion mutant	does not bind	NULL		JNK binding domain		JNK	NULL				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5383_1671_s_95	9733513	A mutated JIP-1 molecule with an in-frame deletion of the JNK binding domain did not bind JNK but did bind MKK7, DLK, MLK3, and HPK1 ( Fig. 3A).	bind
45109	2	11246	6	10	NULL	0	NULL	JIP-1 molecule	NULL	deletion mutant	bind	NULL		JNK binding domain		MKK7	NULL				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5383_1671_s_95	9733513	A mutated JIP-1 molecule with an in-frame deletion of the JNK binding domain did not bind JNK but did bind MKK7, DLK, MLK3, and HPK1 ( Fig. 3A).	bind
45110	3	11246	6	10	NULL	0	NULL	JIP-1 molecule	NULL	deletion mutant	bind	NULL		JNK binding domain		DLK	NULL				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5383_1671_s_95	9733513	A mutated JIP-1 molecule with an in-frame deletion of the JNK binding domain did not bind JNK but did bind MKK7, DLK, MLK3, and HPK1 ( Fig. 3A).	bind
45111	4	11246	6	10	NULL	0	NULL	JIP-1 molecule	NULL	deletion mutant	bind	NULL		JNK binding domain		MLK3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5383_1671_s_95	9733513	A mutated JIP-1 molecule with an in-frame deletion of the JNK binding domain did not bind JNK but did bind MKK7, DLK, MLK3, and HPK1 ( Fig. 3A).	bind
45112	5	11246	6	10	NULL	0	NULL	JIP-1 molecule	NULL	deletion mutant	bind	NULL		JNK binding domain		HPK1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_science_281_5383_1671_s_95	9733513	A mutated JIP-1 molecule with an in-frame deletion of the JNK binding domain did not bind JNK but did bind MKK7, DLK, MLK3, and HPK1 ( Fig. 3A).	bind
44908	1	11247	5	NULL	NULL	NULL	NULL	Rb protein	GP	missense mutant	does not bind			C706F		E1A	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_21_11866_s_180	10518542	A mutated Rb protein carrying a C706F missense mutation which does not bind to oncoproteins E1A and large T antigen but does bind to c- myc and L- myc ( 18) also bound to GST-R-K (Fig.  6 C).	bind
44909	2	11247	5	NULL	NULL	NULL	NULL	E1A	GP		is a type of					oncoprotein	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_21_11866_s_180	10518542	A mutated Rb protein carrying a C706F missense mutation which does not bind to oncoproteins E1A and large T antigen but does bind to c- myc and L- myc ( 18) also bound to GST-R-K (Fig.  6 C).	bind
44910	3	11247	5	NULL	NULL	NULL	NULL	Rb protein	GP	missense mutant	does not bind			C706F		large T antigen	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_21_11866_s_180	10518542	A mutated Rb protein carrying a C706F missense mutation which does not bind to oncoproteins E1A and large T antigen but does bind to c- myc and L- myc ( 18) also bound to GST-R-K (Fig.  6 C).	bind
44911	4	11247	5	NULL	NULL	NULL	NULL	Rb protein	GP	missense mutant	bind			C706F		c- myc	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_21_11866_s_180	10518542	A mutated Rb protein carrying a C706F missense mutation which does not bind to oncoproteins E1A and large T antigen but does bind to c- myc and L- myc ( 18) also bound to GST-R-K (Fig.  6 C).	bind
44912	5	11247	5	NULL	NULL	NULL	NULL	Rb protein	GP	missense mutant	bind			C706F		L- myc	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_21_11866_s_180	10518542	A mutated Rb protein carrying a C706F missense mutation which does not bind to oncoproteins E1A and large T antigen but does bind to c- myc and L- myc ( 18) also bound to GST-R-K (Fig.  6 C).	bind
44913	6	11247	5	NULL	NULL	NULL	NULL	Rb protein	GP	missense mutant	bind			C706F		GST-R-K	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_21_11866_s_180	10518542	A mutated Rb protein carrying a C706F missense mutation which does not bind to oncoproteins E1A and large T antigen but does bind to c- myc and L- myc ( 18) also bound to GST-R-K (Fig.  6 C).	bind
45113	1	11247	6	10	NULL	0	NULL	Rb protein	NULL	missense mutant	does not bind	NULL		C706F		E1A 	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_21_11866_s_180	10518542	A mutated Rb protein carrying a C706F missense mutation which does not bind to oncoproteins E1A and large T antigen but does bind to c- myc and L- myc ( 18) also bound to GST-R-K (Fig.  6 C).	bind
45114	2	11247	6	10	NULL	0	NULL	Rb protein	NULL	missense mutant	does not bind	NULL		C706F		large T antigen	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_21_11866_s_180	10518542	A mutated Rb protein carrying a C706F missense mutation which does not bind to oncoproteins E1A and large T antigen but does bind to c- myc and L- myc ( 18) also bound to GST-R-K (Fig.  6 C).	bind
45115	3	11247	6	10	NULL	0	NULL	Rb protein	NULL	missense mutant	bind	NULL		C706F		c-myc	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_21_11866_s_180	10518542	A mutated Rb protein carrying a C706F missense mutation which does not bind to oncoproteins E1A and large T antigen but does bind to c- myc and L- myc ( 18) also bound to GST-R-K (Fig.  6 C).	bind
45116	4	11247	6	10	NULL	0	NULL	Rb protein	NULL	missense mutant	bind	NULL		C706F		L-myc	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_21_11866_s_180	10518542	A mutated Rb protein carrying a C706F missense mutation which does not bind to oncoproteins E1A and large T antigen but does bind to c- myc and L- myc ( 18) also bound to GST-R-K (Fig.  6 C).	bind
45117	5	11247	6	10	NULL	0	NULL	Rb protein	NULL	missense mutant	bind	NULL		C706F		GST-R-K	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_96_21_11866_s_180	10518542	A mutated Rb protein carrying a C706F missense mutation which does not bind to oncoproteins E1A and large T antigen but does bind to c- myc and L- myc ( 18) also bound to GST-R-K (Fig.  6 C).	bind
45118	6	11247	6	NULL	NULL	0	NULL	E1A	NULL		is a type of	NULL				oncoprotein	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_96_21_11866_s_180	10518542	A mutated Rb protein carrying a C706F missense mutation which does not bind to oncoproteins E1A and large T antigen but does bind to c- myc and L- myc ( 18) also bound to GST-R-K (Fig.  6 C).	bind
44914	1	11248	5	NULL	NULL	NULL	NULL			mutant	does not bind				CGCT CAC CAGCCGC	LHX9	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_14_1839_s_169	12130543	A mutated sequence CGCT CAC CAGCCGC was no longer bound by LHX9.	bind
45119	1	11248	6	NULL	NULL	0	NULL		NULL	mutant	does not bind	NULL			CGCT CAC CAGCCGC	LHX9	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_16_14_1839_s_169	12130543	A mutated sequence CGCT CAC CAGCCGC was no longer bound by LHX9.	bind
44915	1	11249	5	NULL	NULL	NULL	NULL	DAT	GP	mutant	impairs			C terminus		CaMKIIalpha	GP	binding of			NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_neuron_51_4_16908408_s_7	16908408	A mutation  of the DAT C terminus impairing CaMKIIalpha binding also impaired amphetamine-induced  dopamine efflux.	bind
44916	2	11249	5	NULL	NULL	NULL	NULL	amphetamine	Chemical		induce					dopamine efflux	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_neuron_51_4_16908408_s_7	16908408	A mutation  of the DAT C terminus impairing CaMKIIalpha binding also impaired amphetamine-induced  dopamine efflux.	bind
44917	3	11249	5	NULL	NULL	NULL	NULL	DAT	GP	mutant	impairs			C terminus		statement 2	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_neuron_51_4_16908408_s_7	16908408	A mutation  of the DAT C terminus impairing CaMKIIalpha binding also impaired amphetamine-induced  dopamine efflux.	bind
45120	1	11249	6	NULL	NULL	0	NULL	amphetamine	NULL		induces	NULL				dopamine efflux	NULL				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_neuron_51_4_16908408_s_7	16908408	A mutation  of the DAT C terminus impairing CaMKIIalpha binding also impaired amphetamine-induced  dopamine efflux.	bind
45121	2	11249	6	NULL	NULL	0	NULL	DAT	NULL	mutant	impairs	NULL		C terminus		statement 1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_neuron_51_4_16908408_s_7	16908408	A mutation  of the DAT C terminus impairing CaMKIIalpha binding also impaired amphetamine-induced  dopamine efflux.	bind
45122	3	11249	6	NULL	NULL	0	NULL	DAT	NULL	mutant	impairs	NULL		C terminus		CaMKIIalpha	NULL	binding of			NULL		0	NULL	NULL	NULL	abs-batch0740-0759_neuron_51_4_16908408_s_7	16908408	A mutation  of the DAT C terminus impairing CaMKIIalpha binding also impaired amphetamine-induced  dopamine efflux.	bind
44918	2	11250	5	NULL	NULL	NULL	NULL	Prp16	GP	mutant	inhibit			ATP-binding motif		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_8_441_s_9	9550699	A mutation ( prp16-1) near the ATP-binding motif of Prp16 inhibits both the RNA-dependent ATPase activity and the ATP-dependent RNA unwinding activity.	bind
44919	4	11250	5	NULL	NULL	NULL	NULL	Prp16	GP	mutant	inhibit			ATP-binding motif		statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_8_441_s_9	9550699	A mutation ( prp16-1) near the ATP-binding motif of Prp16 inhibits both the RNA-dependent ATPase activity and the ATP-dependent RNA unwinding activity.	bind
45560	1	11250	5	NULL	NULL	NULL	NULL	ATPase activity	Process		is dependent on					RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_8_441_s_9	9550699	A mutation ( prp16-1) near the ATP-binding motif of Prp16 inhibits both the RNA-dependent ATPase activity and the ATP-dependent RNA unwinding activity.	bind
45561	3	11250	5	NULL	NULL	NULL	NULL	RNA unwinding activity	Process		is dependent on					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_8_8_441_s_9	9550699	A mutation ( prp16-1) near the ATP-binding motif of Prp16 inhibits both the RNA-dependent ATPase activity and the ATP-dependent RNA unwinding activity.	bind
45123	1	11250	6	NULL	NULL	0	NULL	ATPase activity	NULL		is dependent on	NULL				RNA	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_8_8_441_s_9	9550699	A mutation ( prp16-1) near the ATP-binding motif of Prp16 inhibits both the RNA-dependent ATPase activity and the ATP-dependent RNA unwinding activity.	bind
45124	2	11250	6	NULL	NULL	0	NULL	RNA unwinding activity	NULL		is dependent on	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_8_8_441_s_9	9550699	A mutation ( prp16-1) near the ATP-binding motif of Prp16 inhibits both the RNA-dependent ATPase activity and the ATP-dependent RNA unwinding activity.	bind
45125	3	11250	6	NULL	NULL	0	NULL	Prp16	NULL	mutant	inhibits	NULL		ATP-binding motif		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_8_8_441_s_9	9550699	A mutation ( prp16-1) near the ATP-binding motif of Prp16 inhibits both the RNA-dependent ATPase activity and the ATP-dependent RNA unwinding activity.	bind
45126	4	11250	6	NULL	NULL	0	NULL	Prp16	NULL	mutant	inhibits	NULL		ATP-binding motif		statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_8_8_441_s_9	9550699	A mutation ( prp16-1) near the ATP-binding motif of Prp16 inhibits both the RNA-dependent ATPase activity and the ATP-dependent RNA unwinding activity.	bind
44920	1	11251	5	NULL	NULL	NULL	NULL	ERalpha537X	GP	mutant	increase					N-CoR	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_6912_s_173	12482846	A Mutation (ERalpha537X) That Increases N-CoR Binding also Inhibits AF-1 Activity-- While SERMs show intriguing effects on ERalpha interactions with N-CoR, it is also clear that these interactions are relatively weak (see "`Discussion"`).	bind
44921	2	11251	5	NULL	NULL	NULL	NULL	ERalpha537X	GP	mutant	inhibit					AF-1 	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_6912_s_173	12482846	A Mutation (ERalpha537X) That Increases N-CoR Binding also Inhibits AF-1 Activity-- While SERMs show intriguing effects on ERalpha interactions with N-CoR, it is also clear that these interactions are relatively weak (see "`Discussion"`).	bind
44922	3	11251	5	NULL	NULL	NULL	NULL	ERalpha	GP		interact with		weakly			N-CoR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_6912_s_173	12482846	A Mutation (ERalpha537X) That Increases N-CoR Binding also Inhibits AF-1 Activity-- While SERMs show intriguing effects on ERalpha interactions with N-CoR, it is also clear that these interactions are relatively weak (see "`Discussion"`).	bind
45127	1	11251	6	NULL	NULL	0	NULL	ERalpha	NULL		interacts with	NULL	weakly			N-CoR	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_6912_s_173	12482846	A Mutation (ERalpha537X) That Increases N-CoR Binding also Inhibits AF-1 Activity-- While SERMs show intriguing effects on ERalpha interactions with N-CoR, it is also clear that these interactions are relatively weak (see "`Discussion"`).	bind
45128	2	11251	6	NULL	NULL	0	NULL	ERalpha537X	NULL	mutant	increases	NULL				N-CoR	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_9_6912_s_173	12482846	A Mutation (ERalpha537X) That Increases N-CoR Binding also Inhibits AF-1 Activity-- While SERMs show intriguing effects on ERalpha interactions with N-CoR, it is also clear that these interactions are relatively weak (see "`Discussion"`).	bind
45129	3	11251	6	NULL	NULL	0	NULL	ERalpha537X	NULL	mutant	inhibits	NULL				AF-1	NULL	activity of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_9_6912_s_173	12482846	A Mutation (ERalpha537X) That Increases N-CoR Binding also Inhibits AF-1 Activity-- While SERMs show intriguing effects on ERalpha interactions with N-CoR, it is also clear that these interactions are relatively weak (see "`Discussion"`).	bind
44923	1	11252	5	NULL	NULL	NULL	NULL	N-CoR	GP		bind					SERMs	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_6912_s_308	12482846	A mutation (L379R) that reduces and equalizes N-CoR binding with SERMs allows equivalent AF-1 activity at simple EREs and AP-1 sites in the presence of SERMs and increases ICI and raloxifene response at C3.	bind
44924	2	11252	5	NULL	NULL	NULL	NULL			mutant	reduces			L379R		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_6912_s_308	12482846	A mutation (L379R) that reduces and equalizes N-CoR binding with SERMs allows equivalent AF-1 activity at simple EREs and AP-1 sites in the presence of SERMs and increases ICI and raloxifene response at C3.	bind
44925	3	11252	5	NULL	NULL	NULL	NULL			mutant	equalizes			L379R		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_6912_s_308	12482846	A mutation (L379R) that reduces and equalizes N-CoR binding with SERMs allows equivalent AF-1 activity at simple EREs and AP-1 sites in the presence of SERMs and increases ICI and raloxifene response at C3.	bind
46383	4	11252	5	NULL	NULL	NULL	NULL			mutant	allows			L379R		AF-1	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_6912_s_308	12482846	A mutation (L379R) that reduces and equalizes N-CoR binding with SERMs allows equivalent AF-1 activity at simple EREs and AP-1 sites in the presence of SERMs and increases ICI and raloxifene response at C3.	bind
46384	5	11252	5	NULL	NULL	NULL	NULL	statement 4	Process		occurs at									EREs	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_6912_s_308	12482846	A mutation (L379R) that reduces and equalizes N-CoR binding with SERMs allows equivalent AF-1 activity at simple EREs and AP-1 sites in the presence of SERMs and increases ICI and raloxifene response at C3.	bind
46385	6	11252	5	NULL	NULL	NULL	NULL	statement 4	Process		occurs at									AP-1 sites	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_6912_s_308	12482846	A mutation (L379R) that reduces and equalizes N-CoR binding with SERMs allows equivalent AF-1 activity at simple EREs and AP-1 sites in the presence of SERMs and increases ICI and raloxifene response at C3.	bind
46386	7	11252	5	NULL	NULL	NULL	NULL	statement 5	Process		is equivalent to					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_6912_s_308	12482846	A mutation (L379R) that reduces and equalizes N-CoR binding with SERMs allows equivalent AF-1 activity at simple EREs and AP-1 sites in the presence of SERMs and increases ICI and raloxifene response at C3.	bind
46387	8	11252	5	NULL	NULL	NULL	NULL	statement 5	Process		in the presence of					SERMs	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_6912_s_308	12482846	A mutation (L379R) that reduces and equalizes N-CoR binding with SERMs allows equivalent AF-1 activity at simple EREs and AP-1 sites in the presence of SERMs and increases ICI and raloxifene response at C3.	bind
46388	9	11252	5	NULL	NULL	NULL	NULL	statement 6	Process		in the presence of					SERMs	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_6912_s_308	12482846	A mutation (L379R) that reduces and equalizes N-CoR binding with SERMs allows equivalent AF-1 activity at simple EREs and AP-1 sites in the presence of SERMs and increases ICI and raloxifene response at C3.	bind
45130	1	11252	6	NULL	NULL	0	NULL	N-CoR	NULL		bind	NULL				SERM	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_9_6912_s_308	12482846	A mutation (L379R) that reduces and equalizes N-CoR binding with SERMs allows equivalent AF-1 activity at simple EREs and AP-1 sites in the presence of SERMs and increases ICI and raloxifene response at C3.	bind
45774	2	11252	6	NULL	NULL	0	NULL		NULL	mutant	reduces	NULL		L379R		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_9_6912_s_308	12482846	A mutation (L379R) that reduces and equalizes N-CoR binding with SERMs allows equivalent AF-1 activity at simple EREs and AP-1 sites in the presence of SERMs and increases ICI and raloxifene response at C3.	bind
45775	3	11252	6	NULL	NULL	0	NULL		NULL	mutant	equalizes	NULL		L379R		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_9_6912_s_308	12482846	A mutation (L379R) that reduces and equalizes N-CoR binding with SERMs allows equivalent AF-1 activity at simple EREs and AP-1 sites in the presence of SERMs and increases ICI and raloxifene response at C3.	bind
45777	4	11252	6	NULL	NULL	0	NULL		NULL	mutant	allows	NULL		L379R		AF-1	NULL	activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_9_6912_s_308	12482846	A mutation (L379R) that reduces and equalizes N-CoR binding with SERMs allows equivalent AF-1 activity at simple EREs and AP-1 sites in the presence of SERMs and increases ICI and raloxifene response at C3.	bind
45778	5	11252	6	NULL	NULL	0	NULL	statement 4	NULL		occurs at	NULL					NULL			ERE	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_9_6912_s_308	12482846	A mutation (L379R) that reduces and equalizes N-CoR binding with SERMs allows equivalent AF-1 activity at simple EREs and AP-1 sites in the presence of SERMs and increases ICI and raloxifene response at C3.	bind
45779	6	11252	6	NULL	NULL	0	NULL	statement 4	NULL		occurs at	NULL					NULL			AP-1 site	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_9_6912_s_308	12482846	A mutation (L379R) that reduces and equalizes N-CoR binding with SERMs allows equivalent AF-1 activity at simple EREs and AP-1 sites in the presence of SERMs and increases ICI and raloxifene response at C3.	bind
45780	7	11252	6	NULL	NULL	0	NULL	statement 5	NULL		occurs in presence of	NULL				SERM	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_9_6912_s_308	12482846	A mutation (L379R) that reduces and equalizes N-CoR binding with SERMs allows equivalent AF-1 activity at simple EREs and AP-1 sites in the presence of SERMs and increases ICI and raloxifene response at C3.	bind
45781	8	11252	6	NULL	NULL	0	NULL	statement 6	NULL		occurs in presence of	NULL				SERM	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_9_6912_s_308	12482846	A mutation (L379R) that reduces and equalizes N-CoR binding with SERMs allows equivalent AF-1 activity at simple EREs and AP-1 sites in the presence of SERMs and increases ICI and raloxifene response at C3.	bind
45212	1	11253	5	NULL	NULL	NULL	NULL	Tfc4	GP		is mutated at					Tfc4	GP		L469K in TPR7		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_40	16880507	A mutation (L469K) in TPR7 of Tfc4, which affects the recruitment of Brf1, also inhibits the direct binding of Bdp1 to Tfc4 and decreases the affinity of Bdp1 for the TBP-Brf1-TFIIIC-DNA complex, suggesting that Brf1 and Bdp1 share an overlapping binding site in Tfc4 ( ).	bind
45213	2	11253	5	NULL	NULL	NULL	NULL	statement 1	Process		affect					Brf1	GP	recruitment of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_40	16880507	A mutation (L469K) in TPR7 of Tfc4, which affects the recruitment of Brf1, also inhibits the direct binding of Bdp1 to Tfc4 and decreases the affinity of Bdp1 for the TBP-Brf1-TFIIIC-DNA complex, suggesting that Brf1 and Bdp1 share an overlapping binding site in Tfc4 ( ).	bind
45214	3	11253	5	NULL	NULL	NULL	NULL	Bdp1	GP		bind		directly			Tfc4	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_40	16880507	A mutation (L469K) in TPR7 of Tfc4, which affects the recruitment of Brf1, also inhibits the direct binding of Bdp1 to Tfc4 and decreases the affinity of Bdp1 for the TBP-Brf1-TFIIIC-DNA complex, suggesting that Brf1 and Bdp1 share an overlapping binding site in Tfc4 ( ).	bind
45215	4	11253	5	NULL	NULL	NULL	NULL	statement 1	Process		inhibit					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_40	16880507	A mutation (L469K) in TPR7 of Tfc4, which affects the recruitment of Brf1, also inhibits the direct binding of Bdp1 to Tfc4 and decreases the affinity of Bdp1 for the TBP-Brf1-TFIIIC-DNA complex, suggesting that Brf1 and Bdp1 share an overlapping binding site in Tfc4 ( ).	bind
45216	5	11253	5	NULL	NULL	NULL	NULL	Bdp1	GP		shows affinity to					TBP-Brf1-TFIIIC-DNA complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_40	16880507	A mutation (L469K) in TPR7 of Tfc4, which affects the recruitment of Brf1, also inhibits the direct binding of Bdp1 to Tfc4 and decreases the affinity of Bdp1 for the TBP-Brf1-TFIIIC-DNA complex, suggesting that Brf1 and Bdp1 share an overlapping binding site in Tfc4 ( ).	bind
45217	6	11253	5	NULL	NULL	NULL	NULL	statement 1	Process		decrease					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_40	16880507	A mutation (L469K) in TPR7 of Tfc4, which affects the recruitment of Brf1, also inhibits the direct binding of Bdp1 to Tfc4 and decreases the affinity of Bdp1 for the TBP-Brf1-TFIIIC-DNA complex, suggesting that Brf1 and Bdp1 share an overlapping binding site in Tfc4 ( ).	bind
45218	7	11253	5	NULL	NULL	NULL	NULL	Brf1	GP		bind					Tfc4	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_40	16880507	A mutation (L469K) in TPR7 of Tfc4, which affects the recruitment of Brf1, also inhibits the direct binding of Bdp1 to Tfc4 and decreases the affinity of Bdp1 for the TBP-Brf1-TFIIIC-DNA complex, suggesting that Brf1 and Bdp1 share an overlapping binding site in Tfc4 ( ).	bind
45219	8	11253	5	NULL	NULL	NULL	NULL	statement 3	Process		overlaps			binding site		statement 7	Process		binding site		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_40	16880507	A mutation (L469K) in TPR7 of Tfc4, which affects the recruitment of Brf1, also inhibits the direct binding of Bdp1 to Tfc4 and decreases the affinity of Bdp1 for the TBP-Brf1-TFIIIC-DNA complex, suggesting that Brf1 and Bdp1 share an overlapping binding site in Tfc4 ( ).	bind
45782	1	11253	6	NULL	NULL	0	NULL	Bdp1	NULL		bind	NULL				Tfc4	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_40	16880507	A mutation (L469K) in TPR7 of Tfc4, which affects the recruitment of Brf1, also inhibits the direct binding of Bdp1 to Tfc4 and decreases the affinity of Bdp1 for the TBP-Brf1-TFIIIC-DNA complex, suggesting that Brf1 and Bdp1 share an overlapping binding site in Tfc4 ( ).	bind
45783	2	11253	6	NULL	NULL	0	NULL	Bdp1	NULL		has affinity for	NULL				TBP-Brf1-TFIIIC-DNA complex	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_40	16880507	A mutation (L469K) in TPR7 of Tfc4, which affects the recruitment of Brf1, also inhibits the direct binding of Bdp1 to Tfc4 and decreases the affinity of Bdp1 for the TBP-Brf1-TFIIIC-DNA complex, suggesting that Brf1 and Bdp1 share an overlapping binding site in Tfc4 ( ).	bind
45784	3	11253	6	NULL	NULL	0	NULL	Tcf4	NULL	mutant	affects	NULL		L469K in TPR7		Brf1	NULL	recruitment of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_40	16880507	A mutation (L469K) in TPR7 of Tfc4, which affects the recruitment of Brf1, also inhibits the direct binding of Bdp1 to Tfc4 and decreases the affinity of Bdp1 for the TBP-Brf1-TFIIIC-DNA complex, suggesting that Brf1 and Bdp1 share an overlapping binding site in Tfc4 ( ).	bind
45785	4	11253	6	NULL	NULL	0	NULL	Tfc4	NULL	mutant	inhibits	NULL		L469K in TPR7		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_40	16880507	A mutation (L469K) in TPR7 of Tfc4, which affects the recruitment of Brf1, also inhibits the direct binding of Bdp1 to Tfc4 and decreases the affinity of Bdp1 for the TBP-Brf1-TFIIIC-DNA complex, suggesting that Brf1 and Bdp1 share an overlapping binding site in Tfc4 ( ).	bind
45786	5	11253	6	NULL	NULL	0	NULL	Tfc4	NULL	mutant	decreases	NULL		L469K in TPR7		statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_16_5946_s_40	16880507	A mutation (L469K) in TPR7 of Tfc4, which affects the recruitment of Brf1, also inhibits the direct binding of Bdp1 to Tfc4 and decreases the affinity of Bdp1 for the TBP-Brf1-TFIIIC-DNA complex, suggesting that Brf1 and Bdp1 share an overlapping binding site in Tfc4 ( ).	bind
45220	1	11254	5	NULL	NULL	NULL	NULL	NOXO1	GP		activates					ROS	GP	generation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_6_4737_s_146	14617635	A Mutation Affecting Lipid Binding Decreases the Ability of NOXO1 to Activate ROS Generation -- Cells were co-transfected with empty vector or plasmid encoding Nox1, NOXA1, plus either NOXO1 or NOXO1(R40Q).	bind
45221	2	11254	5	NULL	NULL	NULL	NULL	mutation 	Process		affect					lipid	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_6_4737_s_146	14617635	A Mutation Affecting Lipid Binding Decreases the Ability of NOXO1 to Activate ROS Generation -- Cells were co-transfected with empty vector or plasmid encoding Nox1, NOXA1, plus either NOXO1 or NOXO1(R40Q).	bind
45222	3	11254	5	NULL	NULL	NULL	NULL	statement 2	Process		decrease					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_6_4737_s_146	14617635	A Mutation Affecting Lipid Binding Decreases the Ability of NOXO1 to Activate ROS Generation -- Cells were co-transfected with empty vector or plasmid encoding Nox1, NOXA1, plus either NOXO1 or NOXO1(R40Q).	bind
45787	1	11254	6	NULL	NULL	0	NULL	NOXO1	NULL		activates	NULL				ROS	NULL	generation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_6_4737_s_146	14617635	A Mutation Affecting Lipid Binding Decreases the Ability of NOXO1 to Activate ROS Generation -- Cells were co-transfected with empty vector or plasmid encoding Nox1, NOXA1, plus either NOXO1 or NOXO1(R40Q).	bind
51247	2	11254	6	10	NULL	0	NULL	mutation 	NULL		affect	NULL				lipid	NULL	binding of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_6_4737_s_146	14617635	A Mutation Affecting Lipid Binding Decreases the Ability of NOXO1 to Activate ROS Generation -- Cells were co-transfected with empty vector or plasmid encoding Nox1, NOXA1, plus either NOXO1 or NOXO1(R40Q).	bind
51248	3	11254	6	10	NULL	0	NULL	statement 2	NULL		decrease	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_6_4737_s_146	14617635	A Mutation Affecting Lipid Binding Decreases the Ability of NOXO1 to Activate ROS Generation -- Cells were co-transfected with empty vector or plasmid encoding Nox1, NOXA1, plus either NOXO1 or NOXO1(R40Q).	bind
45224	1	11255	5	NULL	NULL	NULL	NULL	STAT1	GP		bind					STAT3	GP				NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_66_6_1719_s_9	15448191	A mutation analysis of the 5''- TTCATG GAA-3'' STAT1/3 element (palindrome underlined) was performed to determine nucleotide residues that are necessary for the binding of STAT1 and STAT3.	bind
45788	1	11255	6	NULL	NULL	0	NULL	STAT1	NULL		bind	NULL				STAT3	NULL				NULL		0	NULL	NULL	NULL	gw70_molpharmacol_66_6_1719_s_9	15448191	A mutation analysis of the 5''- TTCATG GAA-3'' STAT1/3 element (palindrome underlined) was performed to determine nucleotide residues that are necessary for the binding of STAT1 and STAT3.	bind
45226	1	11256	5	NULL	NULL	NULL	NULL	apoE molecule	GP		bind					VLDL receptor	GP				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_46_8_1721_s_219	15863833	A mutation at arginine 145 (R145C) partially inhibited the binding of the apoE molecule to the VLDL receptor but completely prevented monoclonal antibody 1D7 from binding.	bind
45227	2	11256	5	NULL	NULL	NULL	NULL			mutant	inhibit		partially	R145C		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_46_8_1721_s_219	15863833	A mutation at arginine 145 (R145C) partially inhibited the binding of the apoE molecule to the VLDL receptor but completely prevented monoclonal antibody 1D7 from binding.	bind
45231	3	11256	5	NULL	NULL	NULL	NULL			mutant	prevents		completely	R145C		1D7	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_46_8_1721_s_219	15863833	A mutation at arginine 145 (R145C) partially inhibited the binding of the apoE molecule to the VLDL receptor but completely prevented monoclonal antibody 1D7 from binding.	bind
45232	4	11256	5	NULL	NULL	NULL	NULL	1D7	GP		is a type of					monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_46_8_1721_s_219	15863833	A mutation at arginine 145 (R145C) partially inhibited the binding of the apoE molecule to the VLDL receptor but completely prevented monoclonal antibody 1D7 from binding.	bind
45789	1	11256	6	NULL	NULL	0	NULL	apoE molecule	NULL		bind	NULL				VLDL receptor	NULL				NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_8_1721_s_219	15863833	A mutation at arginine 145 (R145C) partially inhibited the binding of the apoE molecule to the VLDL receptor but completely prevented monoclonal antibody 1D7 from binding.	bind
45790	2	11256	6	NULL	NULL	0	NULL		NULL	mutant	inhibits	NULL		arginine 145 (R145C)		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_8_1721_s_219	15863833	A mutation at arginine 145 (R145C) partially inhibited the binding of the apoE molecule to the VLDL receptor but completely prevented monoclonal antibody 1D7 from binding.	bind
45791	3	11256	6	NULL	NULL	0	NULL	1D7	NULL		is a type of	NULL				monoclonal antibody	NULL				NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_8_1721_s_219	15863833	A mutation at arginine 145 (R145C) partially inhibited the binding of the apoE molecule to the VLDL receptor but completely prevented monoclonal antibody 1D7 from binding.	bind
45792	4	11256	6	NULL	NULL	0	NULL		NULL	mutant	prevents	NULL		arginine 145 (R145C)		statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_8_1721_s_219	15863833	A mutation at arginine 145 (R145C) partially inhibited the binding of the apoE molecule to the VLDL receptor but completely prevented monoclonal antibody 1D7 from binding.	bind
45233	1	11257	5	NULL	NULL	NULL	NULL	Pto	GP		bind					Pti1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_10_2257_s_310	10811617	A mutation at this residue increases the binding affinity of Pto for Pti1, while it reduces the interaction of Pto with Pti3 and Pti10.	bind
45234	2	11257	5	NULL	NULL	NULL	NULL	Pto	GP		interact with					Pti3	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_10_2257_s_310	10811617	A mutation at this residue increases the binding affinity of Pto for Pti1, while it reduces the interaction of Pto with Pti3 and Pti10.	bind
45235	3	11257	5	NULL	NULL	NULL	NULL	Pto	GP		interact with					Pti10	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_10_2257_s_310	10811617	A mutation at this residue increases the binding affinity of Pto for Pti1, while it reduces the interaction of Pto with Pti3 and Pti10.	bind
45794	1	11257	6	NULL	NULL	0	NULL	Pto	NULL		bind	NULL				Pti10	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_19_10_2257_s_310	10811617	A mutation at this residue increases the binding affinity of Pto for Pti1, while it reduces the interaction of Pto with Pti3 and Pti10.	bind
45795	2	11257	6	NULL	NULL	0	NULL	Pto	NULL		has affinity for	NULL				Pti1	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_19_10_2257_s_310	10811617	A mutation at this residue increases the binding affinity of Pto for Pti1, while it reduces the interaction of Pto with Pti3 and Pti10.	bind
45796	3	11257	6	NULL	NULL	0	NULL	Pto	NULL		bind	NULL				Pti3	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_19_10_2257_s_310	10811617	A mutation at this residue increases the binding affinity of Pto for Pti1, while it reduces the interaction of Pto with Pti3 and Pti10.	bind
45237	1	11258	5	NULL	NULL	NULL	NULL	FAK	GP	recombinant	bind					p85	GP		SH2 domain		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_42_26329_s_152	8824286	A mutation converting Tyr-397 to Phe abolished recombinant FAK binding to p85 or its SH2 domains  in vitro.	bind
45238	2	11258	5	NULL	NULL	0	NULL		NULL		is mutated to	NULL		Tyr-397			NULL		Phe		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_42_26329_s_152	8824286	A mutation converting Tyr-397 to Phe abolished recombinant FAK binding to p85 or its SH2 domains  in vitro.	bind
45239	3	11258	5	NULL	NULL	NULL	NULL	statement 2	Process		abolishes					statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_42_26329_s_152	8824286	A mutation converting Tyr-397 to Phe abolished recombinant FAK binding to p85 or its SH2 domains  in vitro.	bind
45797	1	11258	6	NULL	NULL	0	NULL	FAK	NULL	recombinant	bind	NULL				p85	NULL		SH2 domain		NULL	in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_271_42_26329_s_152	8824286	A mutation converting Tyr-397 to Phe abolished recombinant FAK binding to p85 or its SH2 domains  in vitro.	bind
45798	2	11258	6	NULL	NULL	0	NULL		NULL		is converted to	NULL		Tyr-397			NULL		Phe		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_42_26329_s_152	8824286	A mutation converting Tyr-397 to Phe abolished recombinant FAK binding to p85 or its SH2 domains  in vitro.	bind
45799	3	11258	6	NULL	NULL	0	NULL	statement 2	NULL		abolishes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_42_26329_s_152	8824286	A mutation converting Tyr-397 to Phe abolished recombinant FAK binding to p85 or its SH2 domains  in vitro.	bind
45246	1	11259	5	NULL	NULL	NULL	NULL	PAK	GP	activated	rescues					HUVEC	Cell				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_2_361_s_229	16247032	A mutation crippling the CRIB domain (H83/86L) did not impair the ability of activated PAK to rescue HUVEC from contact inhibition, indicating that this effect does not require Rac binding to PAK.	bind
45247	2	11259	5	NULL	NULL	NULL	NULL	HUVEC	Cell		is rescued from					contact inhibition	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_2_361_s_229	16247032	A mutation crippling the CRIB domain (H83/86L) did not impair the ability of activated PAK to rescue HUVEC from contact inhibition, indicating that this effect does not require Rac binding to PAK.	bind
45250	3	11259	5	NULL	NULL	NULL	NULL	Rac	GP		bind					PAK	GP				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_2_361_s_229	16247032	A mutation crippling the CRIB domain (H83/86L) did not impair the ability of activated PAK to rescue HUVEC from contact inhibition, indicating that this effect does not require Rac binding to PAK.	bind
45254	4	11259	5	NULL	NULL	NULL	NULL	PAK	GP	mutant	does not impair			 CRIB domain H83/86L		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_2_361_s_229	16247032	A mutation crippling the CRIB domain (H83/86L) did not impair the ability of activated PAK to rescue HUVEC from contact inhibition, indicating that this effect does not require Rac binding to PAK.	bind
45256	5	11259	5	NULL	NULL	NULL	NULL	statement 1	Process		does not require					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_2_361_s_229	16247032	A mutation crippling the CRIB domain (H83/86L) did not impair the ability of activated PAK to rescue HUVEC from contact inhibition, indicating that this effect does not require Rac binding to PAK.	bind
45800	1	11259	6	NULL	NULL	0	NULL	Rac	NULL		bind	NULL				PAK	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_171_2_361_s_229	16247032	A mutation crippling the CRIB domain (H83/86L) did not impair the ability of activated PAK to rescue HUVEC from contact inhibition, indicating that this effect does not require Rac binding to PAK.	bind
45801	3	11259	6	10	NULL	0	NULL	HUVEC	NULL		rescued from	NULL				contact inhibition	NULL				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_2_361_s_229	16247032	A mutation crippling the CRIB domain (H83/86L) did not impair the ability of activated PAK to rescue HUVEC from contact inhibition, indicating that this effect does not require Rac binding to PAK.	bind
45802	2	11259	6	10	NULL	0	NULL	PAK	NULL	activated	rescue	NULL				HUVEC	NULL				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_2_361_s_229	16247032	A mutation crippling the CRIB domain (H83/86L) did not impair the ability of activated PAK to rescue HUVEC from contact inhibition, indicating that this effect does not require Rac binding to PAK.	bind
45803	4	11259	6	10	NULL	0	NULL		NULL	mutant	does not impair	NULL		CRIB domain (H83/86L)		statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_2_361_s_229	16247032	A mutation crippling the CRIB domain (H83/86L) did not impair the ability of activated PAK to rescue HUVEC from contact inhibition, indicating that this effect does not require Rac binding to PAK.	bind
45804	5	11259	6	10	NULL	0	NULL	statement 2	NULL		does not require	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_171_2_361_s_229	16247032	A mutation crippling the CRIB domain (H83/86L) did not impair the ability of activated PAK to rescue HUVEC from contact inhibition, indicating that this effect does not require Rac binding to PAK.	bind
45257	1	11260	5	NULL	NULL	NULL	NULL	E7	GP		bind					RB	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_virology_204_2_7941347_s_10	7941347	A mutation either at amino acid 24 or 26 which is known to  disrupt the binding of E7 to RB, the retinoblastoma gene product, did  not strongly affect the nuclear localization of the fusion protein, suggesting  that the nuclear transportation of E7 is mostly independent of RB binding.	bind
45258	2	11260	5	NULL	NULL	NULL	NULL			mutation of	disrupt			amino acid 24		statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_virology_204_2_7941347_s_10	7941347	A mutation either at amino acid 24 or 26 which is known to  disrupt the binding of E7 to RB, the retinoblastoma gene product, did  not strongly affect the nuclear localization of the fusion protein, suggesting  that the nuclear transportation of E7 is mostly independent of RB binding.	bind
45259	3	11260	5	NULL	NULL	NULL	NULL			mutation of	disrupt			amino acid 26		statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_virology_204_2_7941347_s_10	7941347	A mutation either at amino acid 24 or 26 which is known to  disrupt the binding of E7 to RB, the retinoblastoma gene product, did  not strongly affect the nuclear localization of the fusion protein, suggesting  that the nuclear transportation of E7 is mostly independent of RB binding.	bind
45260	4	11260	5	NULL	NULL	NULL	NULL	RB	GP		is					retinoblastoma gene product	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_virology_204_2_7941347_s_10	7941347	A mutation either at amino acid 24 or 26 which is known to  disrupt the binding of E7 to RB, the retinoblastoma gene product, did  not strongly affect the nuclear localization of the fusion protein, suggesting  that the nuclear transportation of E7 is mostly independent of RB binding.	bind
45263	5	11260	5	NULL	NULL	NULL	NULL	E7	GP		is transported to					nucleus	CellComponent				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_virology_204_2_7941347_s_10	7941347	A mutation either at amino acid 24 or 26 which is known to  disrupt the binding of E7 to RB, the retinoblastoma gene product, did  not strongly affect the nuclear localization of the fusion protein, suggesting  that the nuclear transportation of E7 is mostly independent of RB binding.	bind
45266	6	11260	5	NULL	NULL	NULL	NULL	statement 5	Process		is independent of					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_virology_204_2_7941347_s_10	7941347	A mutation either at amino acid 24 or 26 which is known to  disrupt the binding of E7 to RB, the retinoblastoma gene product, did  not strongly affect the nuclear localization of the fusion protein, suggesting  that the nuclear transportation of E7 is mostly independent of RB binding.	bind
45809	1	11260	6	NULL	NULL	0	NULL	E7	NULL		bind	NULL				RB	NULL				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_virology_204_2_7941347_s_10	7941347	A mutation either at amino acid 24 or 26 which is known to  disrupt the binding of E7 to RB, the retinoblastoma gene product, did  not strongly affect the nuclear localization of the fusion protein, suggesting  that the nuclear transportation of E7 is mostly independent of RB binding.	bind
45810	2	11260	6	NULL	NULL	0	NULL	RB	NULL		is 	NULL				retinoblastoma gene product	NULL				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_virology_204_2_7941347_s_10	7941347	A mutation either at amino acid 24 or 26 which is known to  disrupt the binding of E7 to RB, the retinoblastoma gene product, did  not strongly affect the nuclear localization of the fusion protein, suggesting  that the nuclear transportation of E7 is mostly independent of RB binding.	bind
45812	4	11260	6	NULL	NULL	0	NULL	E7	NULL		is transported to	NULL				nucleus	NULL				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_virology_204_2_7941347_s_10	7941347	A mutation either at amino acid 24 or 26 which is known to  disrupt the binding of E7 to RB, the retinoblastoma gene product, did  not strongly affect the nuclear localization of the fusion protein, suggesting  that the nuclear transportation of E7 is mostly independent of RB binding.	bind
45813	5	11260	6	NULL	NULL	0	NULL	statement 4	NULL		is independent of	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_virology_204_2_7941347_s_10	7941347	A mutation either at amino acid 24 or 26 which is known to  disrupt the binding of E7 to RB, the retinoblastoma gene product, did  not strongly affect the nuclear localization of the fusion protein, suggesting  that the nuclear transportation of E7 is mostly independent of RB binding.	bind
51251	6	11260	6	10	NULL	0	NULL		NULL	mutant	disrupt	NULL		amino acid 26		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_virology_204_2_7941347_s_10	7941347	A mutation either at amino acid 24 or 26 which is known to  disrupt the binding of E7 to RB, the retinoblastoma gene product, did  not strongly affect the nuclear localization of the fusion protein, suggesting  that the nuclear transportation of E7 is mostly independent of RB binding.	bind
45267	1	11261	5	NULL	NULL	NULL	NULL	Gem	GP	mouse	is mutated to			tryptophan 269		Gem	GP	mouse	glycine		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_2_651_s_186	14701738	A mutation from tryptophan to glycine at position 269 in mouse Gem (or the equivalent position 270 in human Gem) within the helix that binds calmodulin inhibits its binding.	bind
45268	2	11261	5	NULL	NULL	NULL	NULL	Gem	GP	mouse	bind			tryptophan 269		calmodulin	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_2_651_s_186	14701738	A mutation from tryptophan to glycine at position 269 in mouse Gem (or the equivalent position 270 in human Gem) within the helix that binds calmodulin inhibits its binding.	bind
45269	3	11261	5	NULL	NULL	NULL	NULL	statement 1	Process		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_2_651_s_186	14701738	A mutation from tryptophan to glycine at position 269 in mouse Gem (or the equivalent position 270 in human Gem) within the helix that binds calmodulin inhibits its binding.	bind
45270	4	11261	5	NULL	NULL	NULL	NULL	Gem	GP	mouse	is equivalent to			tryptophan 269		Gem	GP	human	tryptophan 270		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_2_651_s_186	14701738	A mutation from tryptophan to glycine at position 269 in mouse Gem (or the equivalent position 270 in human Gem) within the helix that binds calmodulin inhibits its binding.	bind
45814	1	11261	6	NULL	NULL	0	NULL	Gem	NULL	mouse	bind	NULL		tryptophan 269		calmodulin	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_2_651_s_186	14701738	A mutation from tryptophan to glycine at position 269 in mouse Gem (or the equivalent position 270 in human Gem) within the helix that binds calmodulin inhibits its binding.	bind
45815	2	11261	6	NULL	NULL	0	NULL	Gem	NULL		is changed to	NULL		tryptophan 269		Gem	NULL		glycine 269		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_2_651_s_186	14701738	A mutation from tryptophan to glycine at position 269 in mouse Gem (or the equivalent position 270 in human Gem) within the helix that binds calmodulin inhibits its binding.	bind
45816	3	11261	6	10	NULL	0	NULL	statement 2	NULL		inhibit	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_2_651_s_186	14701738	A mutation from tryptophan to glycine at position 269 in mouse Gem (or the equivalent position 270 in human Gem) within the helix that binds calmodulin inhibits its binding.	bind
45817	4	11261	6	NULL	NULL	0	NULL	Gem	NULL	mouse	is equivalent to	NULL		tryptophan 269		Gem	NULL	human	tryptophan 270		NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_2_651_s_186	14701738	A mutation from tryptophan to glycine at position 269 in mouse Gem (or the equivalent position 270 in human Gem) within the helix that binds calmodulin inhibits its binding.	bind
45271	1	11262	5	NULL	NULL	NULL	NULL	hns	GP		is a type of					global regulatory factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_22_2645_s_61	16291643	A mutation in  hns, a global regulatory factor that regulates many virulence factors, causes a threefold increase in  E. coli vesicle production (Horstman and Kuehn 2002 ).	bind
45272	2	11262	5	NULL	NULL	NULL	NULL	hns	GP		regulates					virulence factors	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_22_2645_s_61	16291643	A mutation in  hns, a global regulatory factor that regulates many virulence factors, causes a threefold increase in  E. coli vesicle production (Horstman and Kuehn 2002 ).	bind
45273	3	11262	5	NULL	NULL	NULL	NULL	hns	GP	mutant	increases					vesicle	CellComponent	E. coli;; production of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_22_2645_s_61	16291643	A mutation in  hns, a global regulatory factor that regulates many virulence factors, causes a threefold increase in  E. coli vesicle production (Horstman and Kuehn 2002 ).	bind
45818	1	11262	6	10	NULL	0	NULL	hns	NULL		is a type of	NULL				global regulatory factor	NULL				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_22_2645_s_61	16291643	A mutation in  hns, a global regulatory factor that regulates many virulence factors, causes a threefold increase in  E. coli vesicle production (Horstman and Kuehn 2002 ).	bind
45819	2	11262	6	NULL	NULL	0	NULL	statement 1	NULL		regulates	NULL				virulence factors	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_22_2645_s_61	16291643	A mutation in  hns, a global regulatory factor that regulates many virulence factors, causes a threefold increase in  E. coli vesicle production (Horstman and Kuehn 2002 ).	bind
45820	3	11262	6	10	NULL	0	NULL	hns	NULL	mutant	increases	NULL				vesicle	NULL	E.coli;;production of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_22_2645_s_61	16291643	A mutation in  hns, a global regulatory factor that regulates many virulence factors, causes a threefold increase in  E. coli vesicle production (Horstman and Kuehn 2002 ).	bind
45274	1	11263	5	NULL	NULL	NULL	NULL	HsdS	GP		bind					HsdM	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_64_2_412_s_344	10839821	A mutation in  hsdS may prevent binding of HsdS to HsdM or, as suggested by Weiserova and Firman ( ), the TRD may influence the precise positioning of HsdR, perhaps in response to the methylation state of the target sequence.	bind
45275	2	11263	5	NULL	NULL	NULL	NULL	hsdS	GP	mutant	prevents		may			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_64_2_412_s_344	10839821	A mutation in  hsdS may prevent binding of HsdS to HsdM or, as suggested by Weiserova and Firman ( ), the TRD may influence the precise positioning of HsdR, perhaps in response to the methylation state of the target sequence.	bind
45276	3	11263	5	NULL	NULL	NULL	NULL				influences			TRD		HsdR	GP	precise positioning of			NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_64_2_412_s_344	10839821	A mutation in  hsdS may prevent binding of HsdS to HsdM or, as suggested by Weiserova and Firman ( ), the TRD may influence the precise positioning of HsdR, perhaps in response to the methylation state of the target sequence.	bind
45277	4	11263	5	NULL	NULL	NULL	NULL	statement 3	Process		occur in response to		may			target sequence	NucleicAcid	methylation state of			NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_64_2_412_s_344	10839821	A mutation in  hsdS may prevent binding of HsdS to HsdM or, as suggested by Weiserova and Firman ( ), the TRD may influence the precise positioning of HsdR, perhaps in response to the methylation state of the target sequence.	bind
45821	1	11263	6	NULL	NULL	0	NULL	HsdS	NULL		bind	NULL				HsdM	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_64_2_412_s_344	10839821	A mutation in  hsdS may prevent binding of HsdS to HsdM or, as suggested by Weiserova and Firman ( ), the TRD may influence the precise positioning of HsdR, perhaps in response to the methylation state of the target sequence.	bind
45822	2	11263	6	NULL	NULL	0	NULL	hsdS	NULL	mutant	prevents	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_64_2_412_s_344	10839821	A mutation in  hsdS may prevent binding of HsdS to HsdM or, as suggested by Weiserova and Firman ( ), the TRD may influence the precise positioning of HsdR, perhaps in response to the methylation state of the target sequence.	bind
45823	3	11263	6	10	NULL	0	NULL				influences			TRD		HsdR		positioning of 			NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_64_2_412_s_344	10839821	A mutation in  hsdS may prevent binding of HsdS to HsdM or, as suggested by Weiserova and Firman ( ), the TRD may influence the precise positioning of HsdR, perhaps in response to the methylation state of the target sequence.	bind
45283	1	11266	5	NULL	NULL	NULL	NULL	actin	GP	Saccharomyces cerevisiae;;mutation of	causes			S14A		temperature-sensitive phenotype					NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_12_0_129_s_489	8970724	A mutation in an ATP-binding loop of  Saccharomyces cerevisiae actin (S14A) causes a temperature-sensitive phenotype.	bind
45284	2	11266	5	NULL	NULL	NULL	NULL	actin	GP	Saccharomyces cerevisiae;;mutation of	is present in			S14A		actin	GP	Saccharomyces cerevisiae;;mutant	ATP-binding loop		NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_12_0_129_s_489	8970724	A mutation in an ATP-binding loop of  Saccharomyces cerevisiae actin (S14A) causes a temperature-sensitive phenotype.	bind
45824	1	11266	6	10	NULL	0	NULL	actin	NULL	mutant;; Saccharomyces cerevisiae	causes a	NULL		ATP-binding loop;;S14A		temperature-sensitive phenotype	NULL				NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_12_0_129_s_489	8970724	A mutation in an ATP-binding loop of  Saccharomyces cerevisiae actin (S14A) causes a temperature-sensitive phenotype.	bind
45287	1	11268	5	NULL	NULL	NULL	NULL	Mcm4 protein	GP	mutation of	affect			ATP-binding motif		ssDNA1	NucleicAcid	 binding activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_45_42471_s_25	12207017	A mutation in an ATP-binding motif of the Mcm4 protein affected the ssDNA1 binding activity of the complex and led to moderate inhibition of the DNA helicase activity ( 9).	bind
45288	2	11268	5	NULL	NULL	NULL	NULL	statement 1	Process		leads to					DNA helicase activity	Process	moderate inhibition of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_45_42471_s_25	12207017	A mutation in an ATP-binding motif of the Mcm4 protein affected the ssDNA1 binding activity of the complex and led to moderate inhibition of the DNA helicase activity ( 9).	bind
45825	1	11268	6	NULL	NULL	0	NULL	Mcm4 protein	NULL	mutant	affects	NULL		ATP-binding motif		ssDNA1	NULL	binding activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_45_42471_s_25	12207017	A mutation in an ATP-binding motif of the Mcm4 protein affected the ssDNA1 binding activity of the complex and led to moderate inhibition of the DNA helicase activity ( 9).	bind
45826	2	11268	6	10	NULL	0	NULL	statement 1			leads to					DNA helicase activity		inhibiton of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_45_42471_s_25	12207017	A mutation in an ATP-binding motif of the Mcm4 protein affected the ssDNA1 binding activity of the complex and led to moderate inhibition of the DNA helicase activity ( 9).	bind
45289	1	11269	5	NULL	NULL	NULL	NULL	SULT1A1 probe	NucleicAcid	mutation of	does not change				EBS3	Elf1	GP	binding affinity of			NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_66_6_1690_s_237	15383623	A mutation in EBS3 of the  SULT1A1 probe did not change the binding affinity for Elf1 or Elk1, but compromised binding of the GABP heterodimer.	bind
45290	2	11269	5	NULL	NULL	NULL	NULL	SULT1A1 probe	NucleicAcid	mutation of	does not change				EBS3	Elk1	GP	binding affinity of			NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_66_6_1690_s_237	15383623	A mutation in EBS3 of the  SULT1A1 probe did not change the binding affinity for Elf1 or Elk1, but compromised binding of the GABP heterodimer.	bind
45291	3	11269	5	NULL	NULL	NULL	NULL	SULT1A1 probe	NucleicAcid	mutation of	compromises				EBS3	GABP heterodimer	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_66_6_1690_s_237	15383623	A mutation in EBS3 of the  SULT1A1 probe did not change the binding affinity for Elf1 or Elk1, but compromised binding of the GABP heterodimer.	bind
45827	1	11269	6	10	NULL	0	NULL	SULT1A1 probe		mutant	did not change				EBS3	Elf1		binding affinity of			NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_66_6_1690_s_237	15383623	A mutation in EBS3 of the  SULT1A1 probe did not change the binding affinity for Elf1 or Elk1, but compromised binding of the GABP heterodimer.	bind
45828	2	11269	6	10	NULL	0	NULL	SULT1A1 probe		mutant	did not change				EBS3	Elk1		binding affinity of			NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_66_6_1690_s_237	15383623	A mutation in EBS3 of the  SULT1A1 probe did not change the binding affinity for Elf1 or Elk1, but compromised binding of the GABP heterodimer.	bind
45829	3	11269	6	10	NULL	0	NULL	SULT1A1 probe		mutant	compromises				EBS3	GABP heterodimer		binding of			NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_66_6_1690_s_237	15383623	A mutation in EBS3 of the  SULT1A1 probe did not change the binding affinity for Elf1 or Elk1, but compromised binding of the GABP heterodimer.	bind
45292	1	11270	5	NULL	NULL	NULL	NULL	RNA polymerase holoenzyme	GP	Escherichia coli	bind					DNA	NucleicAcid			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_12_3019_s_873	9620948	A mutation in region 1.1 of sigma sigma 70 affects promoter DNA binding by Escherichia coli RNA polymerase holoenzyme.	bind
45293	2	11270	5	NULL	NULL	NULL	NULL	sigma 70	GP	mutant	affect			region 1.1		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_12_3019_s_873	9620948	A mutation in region 1.1 of sigma sigma 70 affects promoter DNA binding by Escherichia coli RNA polymerase holoenzyme.	bind
46136	1	11270	6	NULL	NULL	0	NULL	RNA polymerase holoenzyme	NULL	E. coli	bind	NULL				DNA	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_12_3019_s_873	9620948	A mutation in region 1.1 of sigma sigma 70 affects promoter DNA binding by Escherichia coli RNA polymerase holoenzyme.	bind
46137	2	11270	6	10	NULL	0	NULL	sigma70	NULL	mutant	affects	NULL		region 1.1		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_12_3019_s_873	9620948	A mutation in region 1.1 of sigma sigma 70 affects promoter DNA binding by Escherichia coli RNA polymerase holoenzyme.	bind
45294	1	11271	5	NULL	NULL	NULL	NULL	RNA polymerase holoenzyme	GP	E. coli	bind					DNA	NucleicAcid			promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_1_221_s_255	10613885	A mutation in region 1.1 of sigma70 affects promoter DNA binding by  E. coli RNA polymerase holoenzyme.	bind
45295	2	11271	5	NULL	NULL	NULL	NULL	sigma70	GP	mutant	affect				region 1.1	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_1_221_s_255	10613885	A mutation in region 1.1 of sigma70 affects promoter DNA binding by  E. coli RNA polymerase holoenzyme.	bind
45830	1	11272	6	NULL	NULL	0	NULL	RNA polymerase holoenzyme	NULL	Escherichia coli	bind	NULL				DNA 	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_1_162_s_548	11114913	A mutation in region 1.1 of sigma70 affects promoter DNA binding by  Escherichia coli RNA polymerase holoenzyme.	bind
45831	2	11272	6	NULL	NULL	0	NULL	sigma70	NULL	mutant	affects	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_1_162_s_548	11114913	A mutation in region 1.1 of sigma70 affects promoter DNA binding by  Escherichia coli RNA polymerase holoenzyme.	bind
45296	1	11274	5	NULL	NULL	NULL	NULL	complex			bind					single-stranded DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8003_s_26	10567526	A mutation in the ATP binding motifs of the Mcm4 protein affected the single-stranded DNA-binding activity of the complex, which moderately inhibited the DNA helicase activity.	bind
45297	2	11274	5	NULL	NULL	NULL	NULL	Mcm4 protein	GP	mutation in	affect			ATP binding motifs		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8003_s_26	10567526	A mutation in the ATP binding motifs of the Mcm4 protein affected the single-stranded DNA-binding activity of the complex, which moderately inhibited the DNA helicase activity.	bind
45298	3	11274	5	NULL	NULL	NULL	NULL	statement 2	Process		inhibit		moderatley			DNA helicase activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8003_s_26	10567526	A mutation in the ATP binding motifs of the Mcm4 protein affected the single-stranded DNA-binding activity of the complex, which moderately inhibited the DNA helicase activity.	bind
45832	1	11274	6	10	NULL	0	NULL	Mcm4 protein		mutant	affects			ATP-binding motif		complex		DNA binding activity of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_12_8003_s_26	10567526	A mutation in the ATP binding motifs of the Mcm4 protein affected the single-stranded DNA-binding activity of the complex, which moderately inhibited the DNA helicase activity.	bind
45833	2	11274	6	NULL	NULL	0	NULL	statement 1	NULL		inhibits	NULL	moderately			DNA helicase activity	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_12_8003_s_26	10567526	A mutation in the ATP binding motifs of the Mcm4 protein affected the single-stranded DNA-binding activity of the complex, which moderately inhibited the DNA helicase activity.	bind
45299	2	11275	5	NULL	NULL	NULL	NULL	p38 subunit	GP	mutation of	does not alter			ATP binding site		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_20_11607_s_7	9751713	A mutation in the ATP binding site of the p38 subunit did not alter the replication activity of hRFC.	bind
58589	1	11275	5	NULL	NULL	NULL	NULL	hRFC	GP		activates					replication	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_20_11607_s_7	9751713	A mutation in the ATP binding site of the p38 subunit did not alter the replication activity of hRFC.	bind
45834	1	11275	6	10	NULL	0	NULL	hRFC			activates					replication					NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_20_11607_s_7	9751713	A mutation in the ATP binding site of the p38 subunit did not alter the replication activity of hRFC.	bind
45835	2	11275	6	10	NULL	0	NULL	p38 subunit		mutant	did not alter			ATP binding site		statement 1					NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_20_11607_s_7	9751713	A mutation in the ATP binding site of the p38 subunit did not alter the replication activity of hRFC.	bind
45302	1	11276	5	NULL	NULL	NULL	NULL	Rhp51	GP		interact with					Rad22	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1724_s_83	11292845	A mutation in the ATP-binding motifs of Rhp51 does not affect its interactions with Rad22 or itself   It has been reported that Rad51 binds to Rad52 and self-assembles ( 41).	bind
45303	2	11276	5	NULL	NULL	NULL	NULL	Rhp51	GP	mutation of	does not affect			ATP-binding motifs		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1724_s_83	11292845	A mutation in the ATP-binding motifs of Rhp51 does not affect its interactions with Rad22 or itself   It has been reported that Rad51 binds to Rad52 and self-assembles ( 41).	bind
45304	3	11276	5	NULL	NULL	NULL	NULL	Rhp51	GP		bind					Rhp51	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1724_s_83	11292845	A mutation in the ATP-binding motifs of Rhp51 does not affect its interactions with Rad22 or itself   It has been reported that Rad51 binds to Rad52 and self-assembles ( 41).	bind
45305	4	11276	5	NULL	NULL	NULL	NULL	Rhp51	GP	mutation of	does not affect			ATP-binding motifs		statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1724_s_83	11292845	A mutation in the ATP-binding motifs of Rhp51 does not affect its interactions with Rad22 or itself   It has been reported that Rad51 binds to Rad52 and self-assembles ( 41).	bind
45306	5	11276	5	NULL	NULL	NULL	NULL	Rad51	GP		bind					Rad52	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1724_s_83	11292845	A mutation in the ATP-binding motifs of Rhp51 does not affect its interactions with Rad22 or itself   It has been reported that Rad51 binds to Rad52 and self-assembles ( 41).	bind
45307	6	11276	5	NULL	NULL	NULL	NULL	statement 5	Process		undergoes					self-assembling	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1724_s_83	11292845	A mutation in the ATP-binding motifs of Rhp51 does not affect its interactions with Rad22 or itself   It has been reported that Rad51 binds to Rad52 and self-assembles ( 41).	bind
45837	1	11276	6	10	NULL	0	NULL	Rhp51	NULL		interact with	NULL				Rad22	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1724_s_83	11292845	A mutation in the ATP-binding motifs of Rhp51 does not affect its interactions with Rad22 or itself   It has been reported that Rad51 binds to Rad52 and self-assembles ( 41).	bind
45838	2	11276	6	NULL	NULL	0	NULL		NULL	mutant	does not affect	NULL		ATP-binding motif		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1724_s_83	11292845	A mutation in the ATP-binding motifs of Rhp51 does not affect its interactions with Rad22 or itself   It has been reported that Rad51 binds to Rad52 and self-assembles ( 41).	bind
45839	5	11276	6	10	NULL	0	NULL	Rad51	NULL		bind	NULL				Rad52	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1724_s_83	11292845	A mutation in the ATP-binding motifs of Rhp51 does not affect its interactions with Rad22 or itself   It has been reported that Rad51 binds to Rad52 and self-assembles ( 41).	bind
45840	6	11276	6	10	NULL	0	NULL	statement 5	NULL		undergoes	NULL				self-assembling	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1724_s_83	11292845	A mutation in the ATP-binding motifs of Rhp51 does not affect its interactions with Rad22 or itself   It has been reported that Rad51 binds to Rad52 and self-assembles ( 41).	bind
51252	3	11276	6	10	NULL	0	NULL	Rhp51	NULL		bind	NULL				Rhp51	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1724_s_83	11292845	A mutation in the ATP-binding motifs of Rhp51 does not affect its interactions with Rad22 or itself   It has been reported that Rad51 binds to Rad52 and self-assembles ( 41).	bind
51253	4	11276	6	10	NULL	0	NULL	Rhp51	NULL	mutant	does not affect	NULL		ATP-binding motif		statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_8_1724_s_83	11292845	A mutation in the ATP-binding motifs of Rhp51 does not affect its interactions with Rad22 or itself   It has been reported that Rad51 binds to Rad52 and self-assembles ( 41).	bind
45308	1	11277	5	NULL	NULL	NULL	NULL	RecD subunit	GP	mutation of	reduces			consensus ATP-binding sequence		RecBCD enzyme	GP	processivity of;;Escherichia coli			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_13_7_890_s_415	10197988	A mutation in the consensus ATP-binding sequence of the RecD subunit reduces the processivity of the RecBCD enzyme from  Escherichia coli.	bind
45841	1	11277	6	10	NULL	0	NULL	RecD subunit	NULL	mutant	reduces	NULL		ATP-binding sequence		RecBCD enzyme	NULL	processivity of ;;Escherichia coli			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_13_7_890_s_415	10197988	A mutation in the consensus ATP-binding sequence of the RecD subunit reduces the processivity of the RecBCD enzyme from  Escherichia coli.	bind
45312	1	11279	5	NULL	NULL	NULL	NULL	Stat 3D	GP		is					mutation in the DNA binding region	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_12_9016_s_288	11114305	A mutation in the DNA binding region ( Stat 3D) as well as substitution of the STAT3 DNA binding region to STAT1 ( Stat 3/1 (D,Linker)) abolished IL-6 induction (Fig.  6).	bind
45313	2	11279	5	NULL	NULL	NULL	NULL	Stat 3D	GP		abolishes					IL-6	GP	induction of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_12_9016_s_288	11114305	A mutation in the DNA binding region ( Stat 3D) as well as substitution of the STAT3 DNA binding region to STAT1 ( Stat 3/1 (D,Linker)) abolished IL-6 induction (Fig.  6).	bind
45314	3	11279	5	NULL	NULL	NULL	NULL	STAT3	GP		is substituted to			DNA binding region		STAT1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_12_9016_s_288	11114305	A mutation in the DNA binding region ( Stat 3D) as well as substitution of the STAT3 DNA binding region to STAT1 ( Stat 3/1 (D,Linker)) abolished IL-6 induction (Fig.  6).	bind
45315	4	11279	5	NULL	NULL	NULL	NULL	statement 3	Process		abolishes					IL-6	GP	induction of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_12_9016_s_288	11114305	A mutation in the DNA binding region ( Stat 3D) as well as substitution of the STAT3 DNA binding region to STAT1 ( Stat 3/1 (D,Linker)) abolished IL-6 induction (Fig.  6).	bind
45842	1	11279	6	NULL	NULL	0	NULL	STAT 3D	NULL		abolishes	NULL		DNA binding region		IL-6	NULL	induction of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_12_9016_s_288	11114305	A mutation in the DNA binding region ( Stat 3D) as well as substitution of the STAT3 DNA binding region to STAT1 ( Stat 3/1 (D,Linker)) abolished IL-6 induction (Fig.  6).	bind
45843	2	11279	6	NULL	NULL	0	NULL	STAT3	NULL		is substituted by	NULL		DNA binding region		STAT1	NULL		Stat 3/1 (D,Linker)		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_12_9016_s_288	11114305	A mutation in the DNA binding region ( Stat 3D) as well as substitution of the STAT3 DNA binding region to STAT1 ( Stat 3/1 (D,Linker)) abolished IL-6 induction (Fig.  6).	bind
45844	3	11279	6	NULL	NULL	0	NULL	statement 2	NULL		abolishes	NULL				IL-6	NULL	induction of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_12_9016_s_288	11114305	A mutation in the DNA binding region ( Stat 3D) as well as substitution of the STAT3 DNA binding region to STAT1 ( Stat 3/1 (D,Linker)) abolished IL-6 induction (Fig.  6).	bind
51254	4	11279	6	10	NULL	0	NULL	Stat 3D	NULL		is	NULL				mutation in the DNA binding region	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_12_9016_s_288	11114305	A mutation in the DNA binding region ( Stat 3D) as well as substitution of the STAT3 DNA binding region to STAT1 ( Stat 3/1 (D,Linker)) abolished IL-6 induction (Fig.  6).	bind
46393	1	11280	5	NULL	NULL	NULL	NULL	TF	GP	mutant	abolishes				Egr-1 binding site in promoter	shear stress	Process	response to			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_2_281_s_158	9974408	A Mutation in the Egr-1 Binding Site in the TF Promoter Abolishes the Response to Shear Stress   To define more precisely the role of Sp1 and Egr-1 in shear stress  trans-activation of the TF promoter, we analyzed the effect of mutations in the overlapping Sp1/Egr-1 binding site that were known to abolish binding of Sp1 and Egr-1 in vitro.	bind
46394	2	11280	5	NULL	NULL	NULL	NULL	Sp1	GP		bind					Egr-1	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_2_281_s_158	9974408	A Mutation in the Egr-1 Binding Site in the TF Promoter Abolishes the Response to Shear Stress   To define more precisely the role of Sp1 and Egr-1 in shear stress  trans-activation of the TF promoter, we analyzed the effect of mutations in the overlapping Sp1/Egr-1 binding site that were known to abolish binding of Sp1 and Egr-1 in vitro.	bind
46395	3	11280	5	NULL	NULL	NULL	NULL			mutant	abolishes				overlapping Sp1/Egr-1 binding site	statement 2	Process				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_2_281_s_158	9974408	A Mutation in the Egr-1 Binding Site in the TF Promoter Abolishes the Response to Shear Stress   To define more precisely the role of Sp1 and Egr-1 in shear stress  trans-activation of the TF promoter, we analyzed the effect of mutations in the overlapping Sp1/Egr-1 binding site that were known to abolish binding of Sp1 and Egr-1 in vitro.	bind
46140	1	11280	6	NULL	NULL	0	NULL	TF	NULL	mutant	abolishes	NULL			egr-1 binding site of promoter	shear stress	NULL	response to			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_2_281_s_158	9974408	A Mutation in the Egr-1 Binding Site in the TF Promoter Abolishes the Response to Shear Stress   To define more precisely the role of Sp1 and Egr-1 in shear stress  trans-activation of the TF promoter, we analyzed the effect of mutations in the overlapping Sp1/Egr-1 binding site that were known to abolish binding of Sp1 and Egr-1 in vitro.	bind
46141	2	11280	6	NULL	NULL	0	NULL	Sp1	NULL		bind	NULL				Egr-1	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_2_281_s_158	9974408	A Mutation in the Egr-1 Binding Site in the TF Promoter Abolishes the Response to Shear Stress   To define more precisely the role of Sp1 and Egr-1 in shear stress  trans-activation of the TF promoter, we analyzed the effect of mutations in the overlapping Sp1/Egr-1 binding site that were known to abolish binding of Sp1 and Egr-1 in vitro.	bind
46142	3	11280	6	10	NULL	0	NULL		NULL	mutant;;  	abolish	NULL			overlapping Sp1/Egr-1 binding site	statement 2	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_2_281_s_158	9974408	A Mutation in the Egr-1 Binding Site in the TF Promoter Abolishes the Response to Shear Stress   To define more precisely the role of Sp1 and Egr-1 in shear stress  trans-activation of the TF promoter, we analyzed the effect of mutations in the overlapping Sp1/Egr-1 binding site that were known to abolish binding of Sp1 and Egr-1 in vitro.	bind
45309	1	11281	5	NULL	NULL	NULL	NULL	cells	Cell		express					ABCA1	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_5_720_s_137	12615680	A mutation in the first intracellular ATP binding domain, however, also appears to impair apoA-I binding to ABCA1-expressing cells.	bind
45310	2	11281	5	NULL	NULL	NULL	NULL	apoA-I	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_5_720_s_137	12615680	A mutation in the first intracellular ATP binding domain, however, also appears to impair apoA-I binding to ABCA1-expressing cells.	bind
45311	3	11281	5	NULL	NULL	NULL	NULL			mutant	impairs			first intracellular ATP binding domain		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_5_720_s_137	12615680	A mutation in the first intracellular ATP binding domain, however, also appears to impair apoA-I binding to ABCA1-expressing cells.	bind
45845	1	11281	6	NULL	NULL	0	NULL	apoA-I	NULL		bind	NULL				ABCA1-expressing cells	NULL				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_5_720_s_137	12615680	A mutation in the first intracellular ATP binding domain, however, also appears to impair apoA-I binding to ABCA1-expressing cells.	bind
45846	2	11281	6	10	NULL	0	NULL		NULL	mutant	impairs	NULL		first intracellular ATP binding domain		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_23_5_720_s_137	12615680	A mutation in the first intracellular ATP binding domain, however, also appears to impair apoA-I binding to ABCA1-expressing cells.	bind
45316	1	11282	5	NULL	NULL	NULL	NULL	NADH:ubiquinone oxidoreductase complex	GP	mutant	increases			NADH-binding subunit		citrate	Chemical	biosynthesis of			NULL		NULL	NULL	NULL	NULL	gw70_annurevplantbiol_52_0_527_s_401	null	A mutation in the gene encoding the NADH-binding subunit of the NADH:ubiquinone  oxidoreductase complex increases citrate biosynthesis and causes a 30-fold increase  in the internal citrate under certain conditions ( 135).	bind
45317	2	11282	5	NULL	NULL	NULL	NULL	statement 1	Process		increases					citrate	Chemical	internal 			NULL		NULL	NULL	NULL	NULL	gw70_annurevplantbiol_52_0_527_s_401	null	A mutation in the gene encoding the NADH-binding subunit of the NADH:ubiquinone  oxidoreductase complex increases citrate biosynthesis and causes a 30-fold increase  in the internal citrate under certain conditions ( 135).	bind
45858	1	11282	6	NULL	NULL	0	NULL	NADH:ubiquinone oxidoreductase complex	NULL	mutant	increases	NULL		NADH-binding subunit		citrate	NULL	biosynthesis of			NULL		0	NULL	NULL	NULL	gw70_annurevplantbiol_52_0_527_s_401	null	A mutation in the gene encoding the NADH-binding subunit of the NADH:ubiquinone  oxidoreductase complex increases citrate biosynthesis and causes a 30-fold increase  in the internal citrate under certain conditions ( 135).	bind
45859	2	11282	6	10	NULL	0	NULL	statement 1			increases					citrate					NULL		NULL	NULL	NULL	NULL	gw70_annurevplantbiol_52_0_527_s_401	null	A mutation in the gene encoding the NADH-binding subunit of the NADH:ubiquinone  oxidoreductase complex increases citrate biosynthesis and causes a 30-fold increase  in the internal citrate under certain conditions ( 135).	bind
45318	1	11283	5	NULL	NULL	NULL	NULL	FtsZ	GP	B. subtilis;;mutant	supress			GTP binding site		minCD phenotype	GP	overexpression of			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_18_5449_s_77	11514533	A mutation in the GTP binding site of  B. subtilis FtsZ suppresses the  minCD overexpression phenotype.	bind
45860	1	11283	6	10	NULL	0	NULL	FtsZ	NULL	B. subtilis;; mutation of	suppresses	NULL		GTP binding site		minCD phenotype	NULL	overexpression of			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_18_5449_s_77	11514533	A mutation in the GTP binding site of  B. subtilis FtsZ suppresses the  minCD overexpression phenotype.	bind
45320	1	11284	5	NULL	NULL	NULL	NULL	eRF3	GP	mutation of	impairs			GTP-binding motifs		eRF1	GP	binding afbility of			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-biol-chem_279_44_15337765_s_7	15337765	A mutation in the GTP-binding  motifs of eRF3 impairs the eRF1-binding ability without altering the Pab1-  or Upf1-binding activity.	bind
45322	2	11284	5	NULL	NULL	NULL	NULL	statement 1	Process		occurs without altering					Pab1	GP	binding activity of			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-biol-chem_279_44_15337765_s_7	15337765	A mutation in the GTP-binding  motifs of eRF3 impairs the eRF1-binding ability without altering the Pab1-  or Upf1-binding activity.	bind
45324	3	11284	5	NULL	NULL	NULL	NULL	statement 1	Process		occurs without altering					 Upf1	GP	binding activity of			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-biol-chem_279_44_15337765_s_7	15337765	A mutation in the GTP-binding  motifs of eRF3 impairs the eRF1-binding ability without altering the Pab1-  or Upf1-binding activity.	bind
45861	1	11284	6	NULL	NULL	0	NULL	eRF3	NULL	mutant	impairs	NULL		GTP-binding motif		eRF1	NULL	binding ability of 			NULL		0	NULL	NULL	NULL	abs-batch0517-0529_j-biol-chem_279_44_15337765_s_7	15337765	A mutation in the GTP-binding  motifs of eRF3 impairs the eRF1-binding ability without altering the Pab1-  or Upf1-binding activity.	bind
45862	2	11284	6	NULL	NULL	0	NULL	statement 1	NULL		occurs without altering	NULL				Pab1 	NULL	binding activity of			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-biol-chem_279_44_15337765_s_7	15337765	A mutation in the GTP-binding  motifs of eRF3 impairs the eRF1-binding ability without altering the Pab1-  or Upf1-binding activity.	bind
45863	3	11284	6	NULL	NULL	0	NULL	statement 1	NULL		occurs without altering	NULL				Upf1	NULL	binding activity of			NULL		0	NULL	NULL	NULL	abs-batch0517-0529_j-biol-chem_279_44_15337765_s_7	15337765	A mutation in the GTP-binding  motifs of eRF3 impairs the eRF1-binding ability without altering the Pab1-  or Upf1-binding activity.	bind
45325	1	11286	5	NULL	NULL	NULL	NULL	androgen receptor	GP	mutation of	affect			ligand binding domain		steroid	GP	binding characteristics of			NULL	human LNCaP cells	NULL	NULL	NULL	NULL	gw60_amjpathol_162_1_233_s_278	12507906	A mutation in the ligand binding domain of the androgen receptor of human LNCaP cells affects steroid binding characteristics and response to anti-androgens.	bind
45326	2	11286	5	NULL	NULL	NULL	NULL	androgen receptor	GP	mutation of	affect			ligand binding domain		anti-androgens	GP	response to			NULL	human LNCaP cells	NULL	NULL	NULL	NULL	gw60_amjpathol_162_1_233_s_278	12507906	A mutation in the ligand binding domain of the androgen receptor of human LNCaP cells affects steroid binding characteristics and response to anti-androgens.	bind
45864	1	11286	6	10	NULL	0	NULL	androgen receptor	NULL	mutant	affects	NULL		ligand binding domain		steroid	NULL	binding of;; characterstic of 			NULL	human LNCaP cells	NULL	NULL	NULL	NULL	gw60_amjpathol_162_1_233_s_278	12507906	A mutation in the ligand binding domain of the androgen receptor of human LNCaP cells affects steroid binding characteristics and response to anti-androgens.	bind
45865	2	11286	6	10	NULL	0	NULL	androgen receptor	NULL	mutant	affects	NULL		ligand binding domain		anti-androgens	NULL	response to			NULL	human LNCaP cells	NULL	NULL	NULL	NULL	gw60_amjpathol_162_1_233_s_278	12507906	A mutation in the ligand binding domain of the androgen receptor of human LNCaP cells affects steroid binding characteristics and response to anti-androgens.	bind
45327	1	11287	5	NULL	NULL	NULL	NULL	GCN2	GP	yeast	bind					tRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_8_1730_s_43	16601681	A mutation in the m2 motif of the HisRS domain in yeast GCN2 strongly decreased  the binding to tRNA, thus making the kinase unable to phosphorylate eIF2alpha in response to amino-acid deprivation (  et al).	bind
45328	2	11287	5	NULL	NULL	NULL	NULL	GCN2	GP	yeast;;mutant	decreases		strongly	m2 motif of HisRS domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_8_1730_s_43	16601681	A mutation in the m2 motif of the HisRS domain in yeast GCN2 strongly decreased  the binding to tRNA, thus making the kinase unable to phosphorylate eIF2alpha in response to amino-acid deprivation (  et al).	bind
45329	3	11287	5	NULL	NULL	NULL	NULL	GCN2	GP		does not phosphorylate					eIF2alpha	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_8_1730_s_43	16601681	A mutation in the m2 motif of the HisRS domain in yeast GCN2 strongly decreased  the binding to tRNA, thus making the kinase unable to phosphorylate eIF2alpha in response to amino-acid deprivation (  et al).	bind
45330	4	11287	5	NULL	NULL	NULL	NULL	statement 3	GP		in response to					amino-acid	AminoAcid	deprivation of			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_8_1730_s_43	16601681	A mutation in the m2 motif of the HisRS domain in yeast GCN2 strongly decreased  the binding to tRNA, thus making the kinase unable to phosphorylate eIF2alpha in response to amino-acid deprivation (  et al).	bind
45331	5	11287	5	NULL	NULL	NULL	NULL	statement 2	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_8_1730_s_43	16601681	A mutation in the m2 motif of the HisRS domain in yeast GCN2 strongly decreased  the binding to tRNA, thus making the kinase unable to phosphorylate eIF2alpha in response to amino-acid deprivation (  et al).	bind
51255	6	11287	5	NULL	NULL	NULL	NULL	GCN2	GP		is a type of					kinase	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_8_1730_s_43	16601681	A mutation in the m2 motif of the HisRS domain in yeast GCN2 strongly decreased  the binding to tRNA, thus making the kinase unable to phosphorylate eIF2alpha in response to amino-acid deprivation (  et al).	bind
46143	1	11287	6	NULL	NULL	0	NULL	GCN2	NULL	yeast	bind	NULL				tRNA	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_25_8_1730_s_43	16601681	A mutation in the m2 motif of the HisRS domain in yeast GCN2 strongly decreased  the binding to tRNA, thus making the kinase unable to phosphorylate eIF2alpha in response to amino-acid deprivation (  et al).	bind
46144	2	11287	6	NULL	NULL	0	NULL	GCN2	NULL	mutant;; yeast	decreases	NULL	strongly	m2 motif of HisRS domain		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_25_8_1730_s_43	16601681	A mutation in the m2 motif of the HisRS domain in yeast GCN2 strongly decreased  the binding to tRNA, thus making the kinase unable to phosphorylate eIF2alpha in response to amino-acid deprivation (  et al).	bind
46145	3	11287	6	NULL	NULL	0	NULL	GCN2	NULL		is a type of	NULL				kinase	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_25_8_1730_s_43	16601681	A mutation in the m2 motif of the HisRS domain in yeast GCN2 strongly decreased  the binding to tRNA, thus making the kinase unable to phosphorylate eIF2alpha in response to amino-acid deprivation (  et al).	bind
46146	4	11287	6	10	NULL	0	NULL	GCN2	NULL		does not phosphorylate	NULL				eIF2alpha	NULL				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_8_1730_s_43	16601681	A mutation in the m2 motif of the HisRS domain in yeast GCN2 strongly decreased  the binding to tRNA, thus making the kinase unable to phosphorylate eIF2alpha in response to amino-acid deprivation (  et al).	bind
46147	5	11287	6	10	NULL	0	NULL	statement 4	NULL		occurs in response to	NULL				amino-acid	NULL	deprivation of			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_8_1730_s_43	16601681	A mutation in the m2 motif of the HisRS domain in yeast GCN2 strongly decreased  the binding to tRNA, thus making the kinase unable to phosphorylate eIF2alpha in response to amino-acid deprivation (  et al).	bind
46148	6	11287	6	NULL	NULL	0	NULL	statement 2	NULL		abolishes	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_25_8_1730_s_43	16601681	A mutation in the m2 motif of the HisRS domain in yeast GCN2 strongly decreased  the binding to tRNA, thus making the kinase unable to phosphorylate eIF2alpha in response to amino-acid deprivation (  et al).	bind
45332	1	11288	5	NULL	NULL	NULL	NULL	MalY	GP	mutation of	results in			pyridoxal phosphate binding site		betaC-S lyase	GP	loss of;; activity of			NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_62_1_204_s_550	9529892	A mutation in the pyridoxal phosphate binding site of MalY was constructed that resulted in the loss of betaC-S lyase activity, even though the protein was still active as a  mal gene repressor.	bind
45333	2	11288	5	NULL	NULL	NULL	NULL	MalY	GP	mutant	is active as			pyridoxal phosphate binding site		mal gene repressor	GP				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_62_1_204_s_550	9529892	A mutation in the pyridoxal phosphate binding site of MalY was constructed that resulted in the loss of betaC-S lyase activity, even though the protein was still active as a  mal gene repressor.	bind
45866	1	11288	6	NULL	NULL	0	NULL	MalY	NULL	mutant	results in	NULL		pyridoxal phosphate binding site		betaC-S lyase activity	NULL	loss of 			NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_62_1_204_s_550	9529892	A mutation in the pyridoxal phosphate binding site of MalY was constructed that resulted in the loss of betaC-S lyase activity, even though the protein was still active as a  mal gene repressor.	bind
51256	2	11288	6	10	NULL	0	NULL	MalY	NULL	mutant	is active as	NULL		pyridoxal phosphate binding site		mal gene repressor	NULL				NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_62_1_204_s_550	9529892	A mutation in the pyridoxal phosphate binding site of MalY was constructed that resulted in the loss of betaC-S lyase activity, even though the protein was still active as a  mal gene repressor.	bind
45334	2	11289	5	NULL	NULL	NULL	NULL	Raf	GP	mutation of	prevents			Ras binding region		statement 1	Process				NULL	Sf9 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_38_23022_s_200	8798490	A mutation in the Ras binding region of Raf prevented the kinase activation of Raf induced by coexpression with Ras in Sf9 cells ( 25).	bind
45335	3	11289	5	NULL	NULL	NULL	NULL	statement 1	Process		induced by					Ras	GP	coexpression with			NULL	Sf9 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_38_23022_s_200	8798490	A mutation in the Ras binding region of Raf prevented the kinase activation of Raf induced by coexpression with Ras in Sf9 cells ( 25).	bind
51257	1	11289	5	NULL	NULL	NULL	NULL	kinase	GP		activates					Raf	GP				NULL	Sf9 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_38_23022_s_200	8798490	A mutation in the Ras binding region of Raf prevented the kinase activation of Raf induced by coexpression with Ras in Sf9 cells ( 25).	bind
46158	1	11289	6	10	NULL	0	NULL	kinase			activates					Raf					NULL	Sf9 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_38_23022_s_200	8798490	A mutation in the Ras binding region of Raf prevented the kinase activation of Raf induced by coexpression with Ras in Sf9 cells ( 25).	bind
46160	2	11289	6	NULL	NULL	0	NULL	statement 1	NULL		occurs after	NULL				Ras	NULL	coexpression with			NULL	Sf9 cells	0	NULL	NULL	NULL	gw60_jbiolchem_271_38_23022_s_200	8798490	A mutation in the Ras binding region of Raf prevented the kinase activation of Raf induced by coexpression with Ras in Sf9 cells ( 25).	bind
46162	3	11289	6	10	NULL	0	NULL	Raf		mutant	prevents			Ras binding region		statement 1					NULL	Sf9 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_38_23022_s_200	8798490	A mutation in the Ras binding region of Raf prevented the kinase activation of Raf induced by coexpression with Ras in Sf9 cells ( 25).	bind
45336	1	11290	5	NULL	NULL	NULL	NULL	p130Cas	GP	mutation of	reduces		significantly	SH3-binding motif		Src 	GP	kinase activity of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_10_8837_s_376	12496276	A mutation in the SH3-binding motif of p130Cas causes significant reduction  in Src kinase activity ( ).	bind
45868	2	11290	6	10	NULL	0	NULL	p130Cas		mutant	reduces		significantly	SH3-binding motif		Src		kinase activity of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_10_8837_s_376	12496276	A mutation in the SH3-binding motif of p130Cas causes significant reduction  in Src kinase activity ( ).	bind
45337	1	11291	5	NULL	NULL	NULL	NULL	STAT1	GP		bind					STAT3	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_278_5337_477_s_154	9334309	A mutation in the STAT DNA-binding sequence that disrupted the binding of STAT1 and STAT3 (Fig.  4D) blocked completely the ability of CNTF to activate GFAP promoter-driven reporter gene expression (Fig.  4C).	bind
45338	2	11291	5	NULL	NULL	NULL	NULL	STAT	GP	mutation of	disrupts			DNA-binding sequence		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_278_5337_477_s_154	9334309	A mutation in the STAT DNA-binding sequence that disrupted the binding of STAT1 and STAT3 (Fig.  4D) blocked completely the ability of CNTF to activate GFAP promoter-driven reporter gene expression (Fig.  4C).	bind
45339	3	11291	5	NULL	NULL	NULL	NULL	CNTF	GP		activates					GFAP 	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw60_science_278_5337_477_s_154	9334309	A mutation in the STAT DNA-binding sequence that disrupted the binding of STAT1 and STAT3 (Fig.  4D) blocked completely the ability of CNTF to activate GFAP promoter-driven reporter gene expression (Fig.  4C).	bind
45340	4	11291	5	NULL	NULL	NULL	NULL	STAT	GP	mutation of	block		completely	DNA-binding sequence		statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_278_5337_477_s_154	9334309	A mutation in the STAT DNA-binding sequence that disrupted the binding of STAT1 and STAT3 (Fig.  4D) blocked completely the ability of CNTF to activate GFAP promoter-driven reporter gene expression (Fig.  4C).	bind
45869	1	11291	6	NULL	NULL	0	NULL	STAT1	NULL		bind	NULL				STAT3	NULL				NULL		0	NULL	NULL	NULL	gw60_science_278_5337_477_s_154	9334309	A mutation in the STAT DNA-binding sequence that disrupted the binding of STAT1 and STAT3 (Fig.  4D) blocked completely the ability of CNTF to activate GFAP promoter-driven reporter gene expression (Fig.  4C).	bind
45870	2	11291	6	10	NULL	0	NULL	STAT		mutant	disrupts			DNA-binding sequence	 	statement 1					NULL		NULL	NULL	NULL	NULL	gw60_science_278_5337_477_s_154	9334309	A mutation in the STAT DNA-binding sequence that disrupted the binding of STAT1 and STAT3 (Fig.  4D) blocked completely the ability of CNTF to activate GFAP promoter-driven reporter gene expression (Fig.  4C).	bind
45871	3	11291	6	NULL	NULL	0	NULL	CNTF	NULL		activates	NULL				GFAP	NULL			promoter	NULL		0	NULL	NULL	NULL	gw60_science_278_5337_477_s_154	9334309	A mutation in the STAT DNA-binding sequence that disrupted the binding of STAT1 and STAT3 (Fig.  4D) blocked completely the ability of CNTF to activate GFAP promoter-driven reporter gene expression (Fig.  4C).	bind
45872	4	11291	6	10	NULL	0	NULL	STAT		mutant	blocks		completely	DNA-binding sequence	 	statement 3					NULL		NULL	NULL	NULL	NULL	gw60_science_278_5337_477_s_154	9334309	A mutation in the STAT DNA-binding sequence that disrupted the binding of STAT1 and STAT3 (Fig.  4D) blocked completely the ability of CNTF to activate GFAP promoter-driven reporter gene expression (Fig.  4C).	bind
45341	1	11292	5	NULL	NULL	NULL	NULL	TFC3	GP	mutation of	decreases			tau138 subunit		TFIIIC-tRNA gene (DNA)	GP	binding affinity of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_1_s_28	9418847	A mutation in the tau138 subunit, encoded by  TFC3, decreased TFIIIC-tRNA gene (DNA) binding affinity and also affected 5S RNA synthesis in vitro ( 34).	bind
45342	2	11292	5	NULL	NULL	NULL	NULL	TFC3	GP	mutation of	affect			tau138 subunit		5S RNA	NucleicAcid	synthesis of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_1_s_28	9418847	A mutation in the tau138 subunit, encoded by  TFC3, decreased TFIIIC-tRNA gene (DNA) binding affinity and also affected 5S RNA synthesis in vitro ( 34).	bind
60554	3	11292	5	NULL	NULL	NULL	NULL	tau138 subunit	GP		is encoded by					TFC3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_1_s_28	9418847	A mutation in the tau138 subunit, encoded by  TFC3, decreased TFIIIC-tRNA gene (DNA) binding affinity and also affected 5S RNA synthesis in vitro ( 34).	bind
45875	1	11292	6	NULL	NULL	0	NULL	tau138 subunit	NULL		is encoded by	NULL				TFC3	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_1_s_28	9418847	A mutation in the tau138 subunit, encoded by  TFC3, decreased TFIIIC-tRNA gene (DNA) binding affinity and also affected 5S RNA synthesis in vitro ( 34).	bind
45876	2	11292	6	10	NULL	0	NULL		NULL	mutant	decreases	NULL		tau138 subunit		TFIIIC-tRNA gene	NULL	binding affinity of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_1_s_28	9418847	A mutation in the tau138 subunit, encoded by  TFC3, decreased TFIIIC-tRNA gene (DNA) binding affinity and also affected 5S RNA synthesis in vitro ( 34).	bind
45877	3	11292	6	10	NULL	0	NULL		NULL	mutant	affects	NULL		tau138 subunit		5S RNA	NULL	synthesis of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_1_s_28	9418847	A mutation in the tau138 subunit, encoded by  TFC3, decreased TFIIIC-tRNA gene (DNA) binding affinity and also affected 5S RNA synthesis in vitro ( 34).	bind
45343	1	11293	5	NULL	NULL	NULL	NULL	PRMT5 construct	GP	myc-tagged;;mutation of	leads to			S-adenosyl-L-methionine-binding motif I		enzymatic activity	Process	near complete loss of			NULL	COS-1 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_35_32971_s_9	11413150	A mutation introduced into the  S-adenosyl-L-methionine-binding motif I of a  myc-tagged PRMT5 construct in COS-1 cells led to a near complete loss of observed enzymatic activity.	bind
45878	1	11293	6	10	NULL	0	NULL	PRMT5 construct	NULL	Myc-tagged;; mutant	leads to	NULL		S-adenosyl-L-methionine-binding motif I		enzymatic activity	NULL	complete loss of			NULL	COS-1 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_35_32971_s_9	11413150	A mutation introduced into the  S-adenosyl-L-methionine-binding motif I of a  myc-tagged PRMT5 construct in COS-1 cells led to a near complete loss of observed enzymatic activity.	bind
45344	1	11294	5	NULL	NULL	NULL	NULL	mTOR	GP		bind					FKBP12-rapamycin complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_2_815_s_243	7822316	A mutation leading to a  reduction in the binding affinity of mTOR for the FKBP12-rapamycin  complex, with otherwise normal mTOR catalytic activity, would be  predicted to act in a dominant fashion in heterozygotes.	bind
45879	1	11294	6	NULL	NULL	0	NULL	mTOR	NULL		bind	NULL				FKBP12-rapamycin complex	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_2_815_s_243	7822316	A mutation leading to a  reduction in the binding affinity of mTOR for the FKBP12-rapamycin  complex, with otherwise normal mTOR catalytic activity, would be  predicted to act in a dominant fashion in heterozygotes.	bind
45347	1	11295	5	NULL	NULL	NULL	NULL	ST	GP		bind					PP2A	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_4_1298_s_161	15684382	A mutation of a cysteine (C103S) that disrupts ST binding to PP2A ( ) resulted in a complete loss of PP2A binding to AR, even upon overexpression of the mutant ST (Fig.  3C).	bind
45348	2	11295	5	NULL	NULL	NULL	NULL			mutant	disrupts			C103S		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_4_1298_s_161	15684382	A mutation of a cysteine (C103S) that disrupts ST binding to PP2A ( ) resulted in a complete loss of PP2A binding to AR, even upon overexpression of the mutant ST (Fig.  3C).	bind
45349	3	11295	5	NULL	NULL	NULL	NULL	PP2A	GP		bind					AR	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_4_1298_s_161	15684382	A mutation of a cysteine (C103S) that disrupts ST binding to PP2A ( ) resulted in a complete loss of PP2A binding to AR, even upon overexpression of the mutant ST (Fig.  3C).	bind
45350	4	11295	5	NULL	NULL	NULL	NULL	statement 2	Process		results in					statement 3	Process	complete loss of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_4_1298_s_161	15684382	A mutation of a cysteine (C103S) that disrupts ST binding to PP2A ( ) resulted in a complete loss of PP2A binding to AR, even upon overexpression of the mutant ST (Fig.  3C).	bind
45351	5	11295	5	NULL	NULL	NULL	NULL	ST	GP	overexpression of;;mutant	results in					statement 3	Process	complete loss of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_4_1298_s_161	15684382	A mutation of a cysteine (C103S) that disrupts ST binding to PP2A ( ) resulted in a complete loss of PP2A binding to AR, even upon overexpression of the mutant ST (Fig.  3C).	bind
45880	1	11295	6	NULL	NULL	0	NULL	ST	NULL		bind	NULL				PP2A	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_4_1298_s_161	15684382	A mutation of a cysteine (C103S) that disrupts ST binding to PP2A ( ) resulted in a complete loss of PP2A binding to AR, even upon overexpression of the mutant ST (Fig.  3C).	bind
45881	2	11295	6	NULL	NULL	0	NULL		NULL	mutant	disrupts	NULL		cysteine;; C103S		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_4_1298_s_161	15684382	A mutation of a cysteine (C103S) that disrupts ST binding to PP2A ( ) resulted in a complete loss of PP2A binding to AR, even upon overexpression of the mutant ST (Fig.  3C).	bind
45882	3	11295	6	NULL	NULL	0	NULL	PP2A	NULL		bind	NULL				AR	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_4_1298_s_161	15684382	A mutation of a cysteine (C103S) that disrupts ST binding to PP2A ( ) resulted in a complete loss of PP2A binding to AR, even upon overexpression of the mutant ST (Fig.  3C).	bind
45883	4	11295	6	NULL	NULL	0	NULL		NULL	mutant	results in	NULL		cysteine;; C103S		statement 3	NULL	complete loss of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_4_1298_s_161	15684382	A mutation of a cysteine (C103S) that disrupts ST binding to PP2A ( ) resulted in a complete loss of PP2A binding to AR, even upon overexpression of the mutant ST (Fig.  3C).	bind
45352	1	11296	5	NULL	NULL	NULL	NULL	ASK1	GP		bind					SOCS1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_9_5559_s_201	16407264	A mutation of ASK1 at Tyr-718 (ASK1-Y718F) diminished the binding to SOCS1 in both assays.	bind
45353	2	11296	5	NULL	NULL	NULL	NULL	ASK1	GP	mutant	diminishes			Y718F		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_9_5559_s_201	16407264	A mutation of ASK1 at Tyr-718 (ASK1-Y718F) diminished the binding to SOCS1 in both assays.	bind
45884	1	11296	6	NULL	NULL	0	NULL	ASK1	NULL		bind	NULL				SOCS1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_9_5559_s_201	16407264	A mutation of ASK1 at Tyr-718 (ASK1-Y718F) diminished the binding to SOCS1 in both assays.	bind
45885	2	11296	6	NULL	NULL	0	NULL	ASK1	NULL	mutant	diminishes	NULL		Tyr-718		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_9_5559_s_201	16407264	A mutation of ASK1 at Tyr-718 (ASK1-Y718F) diminished the binding to SOCS1 in both assays.	bind
45354	1	11297	5	NULL	NULL	NULL	NULL	glycine	AminoAcid		is mutated to			305		arginine	AminoAcid		305		NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1647_1_206_s_75	12686134	A mutation of glycine 305 to arginine will most probably affect cofactor binding  and potentially also the binding of the substrate serine, assuming that serine binds  to CBS in a similar fashion as the substrate analogue methionine in the complex structure  of OASS [  15].	bind
45355	2	11297	5	NULL	NULL	NULL	NULL	statement 1	Process		affect		probably			cofactor	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1647_1_206_s_75	12686134	A mutation of glycine 305 to arginine will most probably affect cofactor binding  and potentially also the binding of the substrate serine, assuming that serine binds  to CBS in a similar fashion as the substrate analogue methionine in the complex structure  of OASS [  15].	bind
45356	3	11297	5	NULL	NULL	NULL	NULL	statement 1	Process		affect		potentially			substrate serine	AminoAcid	binding of			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1647_1_206_s_75	12686134	A mutation of glycine 305 to arginine will most probably affect cofactor binding  and potentially also the binding of the substrate serine, assuming that serine binds  to CBS in a similar fashion as the substrate analogue methionine in the complex structure  of OASS [  15].	bind
45357	4	11297	5	NULL	NULL	NULL	NULL	serine	AminoAcid		bind		may			CBS	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1647_1_206_s_75	12686134	A mutation of glycine 305 to arginine will most probably affect cofactor binding  and potentially also the binding of the substrate serine, assuming that serine binds  to CBS in a similar fashion as the substrate analogue methionine in the complex structure  of OASS [  15].	bind
45886	1	11297	6	NULL	NULL	0	NULL	glycine	NULL		is mutated to	NULL				arginine	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1647_1_206_s_75	12686134	A mutation of glycine 305 to arginine will most probably affect cofactor binding  and potentially also the binding of the substrate serine, assuming that serine binds  to CBS in a similar fashion as the substrate analogue methionine in the complex structure  of OASS [  15].	bind
45887	2	11297	6	NULL	NULL	0	NULL	statement 1	NULL		affects	NULL	probably			cofactor	NULL	binding of			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1647_1_206_s_75	12686134	A mutation of glycine 305 to arginine will most probably affect cofactor binding  and potentially also the binding of the substrate serine, assuming that serine binds  to CBS in a similar fashion as the substrate analogue methionine in the complex structure  of OASS [  15].	bind
45888	3	11297	6	NULL	NULL	0	NULL	statement 1	NULL		affects	NULL				substrate serine	NULL	binding of			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1647_1_206_s_75	12686134	A mutation of glycine 305 to arginine will most probably affect cofactor binding  and potentially also the binding of the substrate serine, assuming that serine binds  to CBS in a similar fashion as the substrate analogue methionine in the complex structure  of OASS [  15].	bind
51274	4	11297	6	10	NULL	0	NULL	serine	NULL		bind	NULL				CBS	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1647_1_206_s_75	12686134	A mutation of glycine 305 to arginine will most probably affect cofactor binding  and potentially also the binding of the substrate serine, assuming that serine binds  to CBS in a similar fashion as the substrate analogue methionine in the complex structure  of OASS [  15].	bind
45360	1	11299	5	NULL	NULL	NULL	NULL	Rad27	GP	mutation of	eliminates					PCNA	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5373_s_38	10409728	A mutation of Rad27 eliminating PCNA binding had very little effect by itself but had major consequences via intragenic or intergenic interactions.	bind
45889	1	11299	6	NULL	NULL	0	NULL	Rad27	NULL	mutant	eliminates	NULL				PCNA	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_8_5373_s_38	10409728	A mutation of Rad27 eliminating PCNA binding had very little effect by itself but had major consequences via intragenic or intergenic interactions.	bind
45361	1	11300	5	NULL	NULL	NULL	NULL	RG2	GP		is					E1A amino terminus	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_cell-growth-differ_7_10_8891337_s_11	8891337	A mutation of the E1A amino terminus  (RG2), which inhibits binding of p300 and related high molecular weight  proteins, reduced 12S repression by 40%.	bind
45362	2	11300	5	NULL	NULL	NULL	NULL	E1A	GP	mutation of	inhibit			RG2		p300	GP	binding of			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_cell-growth-differ_7_10_8891337_s_11	8891337	A mutation of the E1A amino terminus  (RG2), which inhibits binding of p300 and related high molecular weight  proteins, reduced 12S repression by 40%.	bind
51275	3	11300	5	NULL	NULL	NULL	NULL	E1A	GP	mutant	reduce			amino terminus		12S	GP	repression of			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_cell-growth-differ_7_10_8891337_s_11	8891337	A mutation of the E1A amino terminus  (RG2), which inhibits binding of p300 and related high molecular weight  proteins, reduced 12S repression by 40%.	bind
45890	1	11300	6	10	NULL	0	NULL	E1A	NULL	mutant	inhibits	NULL		amino terminus 		p300	NULL	binding of			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_cell-growth-differ_7_10_8891337_s_11	8891337	A mutation of the E1A amino terminus  (RG2), which inhibits binding of p300 and related high molecular weight  proteins, reduced 12S repression by 40%.	bind
45891	2	11300	6	10	NULL	0	NULL	E1A	NULL	mutant	reduces	NULL		amino terminus		12S	NULL	repression of			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_cell-growth-differ_7_10_8891337_s_11	8891337	A mutation of the E1A amino terminus  (RG2), which inhibits binding of p300 and related high molecular weight  proteins, reduced 12S repression by 40%.	bind
51276	3	11300	6	10	NULL	0	NULL	RG2	NULL		is	NULL				E1A amino terminus	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_cell-growth-differ_7_10_8891337_s_11	8891337	A mutation of the E1A amino terminus  (RG2), which inhibits binding of p300 and related high molecular weight  proteins, reduced 12S repression by 40%.	bind
45364	1	11301	5	NULL	NULL	NULL	NULL				is similar to			M875VPM878TLM881		Ctr1	GP	S. cerevisiae	copper-binding motifs		NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_13_3804_s_281	12813074	A mutation of the sequence motif M875VPM878TLM881, which is similar to the copper-binding motifs of Ctr1 and Ctr3 ( S.  cerevisiae) ( ,  ,  ) and Ctr4 ( S.  pombe) ( ), had no influence on copper resistance.	bind
45365	2	11301	5	NULL	NULL	NULL	NULL				is similar to			M875VPM878TLM881		Ctr3	GP	S. cerevisiae	copper-binding motifs		NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_13_3804_s_281	12813074	A mutation of the sequence motif M875VPM878TLM881, which is similar to the copper-binding motifs of Ctr1 and Ctr3 ( S.  cerevisiae) ( ,  ,  ) and Ctr4 ( S.  pombe) ( ), had no influence on copper resistance.	bind
45366	3	11301	5	NULL	NULL	NULL	NULL				is similar to			M875VPM878TLM881		Ctr4	GP	S. pombe	copper-binding motifs		NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_13_3804_s_281	12813074	A mutation of the sequence motif M875VPM878TLM881, which is similar to the copper-binding motifs of Ctr1 and Ctr3 ( S.  cerevisiae) ( ,  ,  ) and Ctr4 ( S.  pombe) ( ), had no influence on copper resistance.	bind
45367	4	11301	5	NULL	NULL	NULL	NULL			mutation of	does not influence			M875VPM878TLM881		copper resistance	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_13_3804_s_281	12813074	A mutation of the sequence motif M875VPM878TLM881, which is similar to the copper-binding motifs of Ctr1 and Ctr3 ( S.  cerevisiae) ( ,  ,  ) and Ctr4 ( S.  pombe) ( ), had no influence on copper resistance.	bind
45894	1	11301	6	10	NULL	0	NULL		NULL	mutant	does not influence	NULL		M875VPM878TLM881		copper resistance	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_13_3804_s_281	12813074	A mutation of the sequence motif M875VPM878TLM881, which is similar to the copper-binding motifs of Ctr1 and Ctr3 ( S.  cerevisiae) ( ,  ,  ) and Ctr4 ( S.  pombe) ( ), had no influence on copper resistance.	bind
45898	3	11301	6	10	NULL	0	NULL		NULL		is similar to	NULL		M875VPM878TLM881		Ctr1	NULL	S. cerevisiae	copper-binding motif		NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_13_3804_s_281	12813074	A mutation of the sequence motif M875VPM878TLM881, which is similar to the copper-binding motifs of Ctr1 and Ctr3 ( S.  cerevisiae) ( ,  ,  ) and Ctr4 ( S.  pombe) ( ), had no influence on copper resistance.	bind
45899	2	11301	6	10	NULL	0	NULL		NULL		is similar to	NULL		M875VPM878TLM881		Ctr4	NULL	 S. pombe	copper-binding motif		NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_13_3804_s_281	12813074	A mutation of the sequence motif M875VPM878TLM881, which is similar to the copper-binding motifs of Ctr1 and Ctr3 ( S.  cerevisiae) ( ,  ,  ) and Ctr4 ( S.  pombe) ( ), had no influence on copper resistance.	bind
45900	4	11301	6	10	NULL	0	NULL		NULL		is similar to	NULL		M875VPM878TLM881		Ctr3	NULL	S. cerevisiae	copper-binding motif		NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_13_3804_s_281	12813074	A mutation of the sequence motif M875VPM878TLM881, which is similar to the copper-binding motifs of Ctr1 and Ctr3 ( S.  cerevisiae) ( ,  ,  ) and Ctr4 ( S.  pombe) ( ), had no influence on copper resistance.	bind
45387	2	11303	5	NULL	NULL	NULL	NULL	Gab1	GP		interacts with					SHP-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_4109_s_8	9632795	A mutation of tyrosine 759, the SHP-2 binding site of gp130, abrogated the interactions of Gab1 with SHP-2 and PI-3 kinase as well as ERK2 activation.	bind
45388	3	11303	5	NULL	NULL	NULL	NULL	Gab1	GP		interacts with					PI-3 kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_4109_s_8	9632795	A mutation of tyrosine 759, the SHP-2 binding site of gp130, abrogated the interactions of Gab1 with SHP-2 and PI-3 kinase as well as ERK2 activation.	bind
45389	4	11303	5	NULL	NULL	NULL	NULL	gp130	GP	mutation of	abrogates			tyrosine 759;;SHP-2 binding site		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_4109_s_8	9632795	A mutation of tyrosine 759, the SHP-2 binding site of gp130, abrogated the interactions of Gab1 with SHP-2 and PI-3 kinase as well as ERK2 activation.	bind
45390	5	11303	5	NULL	NULL	NULL	NULL	gp130	GP	mutation of	abrogates			tyrosine 759;;SHP-2 binding site		statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_4109_s_8	9632795	A mutation of tyrosine 759, the SHP-2 binding site of gp130, abrogated the interactions of Gab1 with SHP-2 and PI-3 kinase as well as ERK2 activation.	bind
45391	1	11303	5	NULL	NULL	NULL	NULL	gp130	GP	mutation of	abrogates			tyrosine 759;;SHP-2 binding site		ERK2	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_4109_s_8	9632795	A mutation of tyrosine 759, the SHP-2 binding site of gp130, abrogated the interactions of Gab1 with SHP-2 and PI-3 kinase as well as ERK2 activation.	bind
45906	1	11303	6	10	NULL	0	NULL	Gab1			interacts with					SHP-2					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_4109_s_8	9632795	A mutation of tyrosine 759, the SHP-2 binding site of gp130, abrogated the interactions of Gab1 with SHP-2 and PI-3 kinase as well as ERK2 activation.	bind
45907	2	11303	6	10	NULL	0	NULL	Gab1			interacts with					PI-3 kinase					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_4109_s_8	9632795	A mutation of tyrosine 759, the SHP-2 binding site of gp130, abrogated the interactions of Gab1 with SHP-2 and PI-3 kinase as well as ERK2 activation.	bind
45908	3	11303	6	10	NULL	0	NULL	gp130	NULL	mutant	abrogates	NULL		tyrosine 759;; the SHP-2 binding site		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_4109_s_8	9632795	A mutation of tyrosine 759, the SHP-2 binding site of gp130, abrogated the interactions of Gab1 with SHP-2 and PI-3 kinase as well as ERK2 activation.	bind
45909	4	11303	6	10	NULL	0	NULL	gp130	NULL	mutant	abrogates	NULL		tyrosine 759;; the SHP-2 binding site		statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_4109_s_8	9632795	A mutation of tyrosine 759, the SHP-2 binding site of gp130, abrogated the interactions of Gab1 with SHP-2 and PI-3 kinase as well as ERK2 activation.	bind
45910	5	11303	6	10	NULL	0	NULL	gp130	NULL	mutant	abrogates	NULL		tyrosine 759;;SHP-2 binding site		ERK2	NULL	activation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_4109_s_8	9632795	A mutation of tyrosine 759, the SHP-2 binding site of gp130, abrogated the interactions of Gab1 with SHP-2 and PI-3 kinase as well as ERK2 activation.	bind
45392	1	11304	5	NULL	NULL	NULL	NULL			mutation of	abolishes		efficiently		GAS element	Stat3	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_517_s_217	11463377	A mutation on both GAS and AP1 elements efficiently abolished the binding of both Stat3 and c-Jun (  Figure 7e, panel II; compare wild type with DM lanes).	bind
45393	2	11304	5	NULL	NULL	NULL	NULL			mutation of	abolishes		efficiently		GAS element	Stat3	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_517_s_217	11463377	A mutation on both GAS and AP1 elements efficiently abolished the binding of both Stat3 and c-Jun (  Figure 7e, panel II; compare wild type with DM lanes).	bind
45394	3	11304	5	NULL	NULL	NULL	NULL			mutation of	abolishes		efficiently		AP1 element	c-Jun	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_517_s_217	11463377	A mutation on both GAS and AP1 elements efficiently abolished the binding of both Stat3 and c-Jun (  Figure 7e, panel II; compare wild type with DM lanes).	bind
45395	4	11304	5	NULL	NULL	NULL	NULL			mutation of	abolishes		efficiently		AP1 element	c-Jun	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_517_s_217	11463377	A mutation on both GAS and AP1 elements efficiently abolished the binding of both Stat3 and c-Jun (  Figure 7e, panel II; compare wild type with DM lanes).	bind
45912	1	11304	6	10	NULL	0	NULL			mutation of	abolishes		efficiently		GAS element	Stat3		binding of 			NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_517_s_217	11463377	A mutation on both GAS and AP1 elements efficiently abolished the binding of both Stat3 and c-Jun (  Figure 7e, panel II; compare wild type with DM lanes).	bind
45913	2	11304	6	10	NULL	0	NULL			mutation of	abolishes		efficiently		GAS element	c-Jun		binding of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_517_s_217	11463377	A mutation on both GAS and AP1 elements efficiently abolished the binding of both Stat3 and c-Jun (  Figure 7e, panel II; compare wild type with DM lanes).	bind
52954	3	11304	6	NULL	NULL	0	NULL		NULL	mutation of	abolishes	NULL	efficiently		AP1 element	Stat3	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_3_517_s_217	11463377	A mutation on both GAS and AP1 elements efficiently abolished the binding of both Stat3 and c-Jun (  Figure 7e, panel II; compare wild type with DM lanes).	bind
52955	4	11304	6	NULL	NULL	0	NULL		NULL	mutation of	abolishes	NULL	efficiently		AP1 element	c-Jun	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_molcell_7_3_517_s_217	11463377	A mutation on both GAS and AP1 elements efficiently abolished the binding of both Stat3 and c-Jun (  Figure 7e, panel II; compare wild type with DM lanes).	bind
46389	1	11305	5	NULL	NULL	NULL	NULL	ets	GP		bind									EBS	NULL		NULL	NULL	NULL	NULL	gw60_gene_307_0_87_s_118	12706891	A mutation that disrupted ets binding to the EBS but retained Sp1 binding at this site as well as disruption of both Sp1 and ets binding to the EBS resulted in comparable inhibition of the promoter activity suggesting that at the EBS the binding of ets alone contributes to the promoter activity.	bind
46390	2	11305	5	NULL	NULL	NULL	NULL	Sp1	GP		bind									EBS	NULL		NULL	NULL	NULL	NULL	gw60_gene_307_0_87_s_118	12706891	A mutation that disrupted ets binding to the EBS but retained Sp1 binding at this site as well as disruption of both Sp1 and ets binding to the EBS resulted in comparable inhibition of the promoter activity suggesting that at the EBS the binding of ets alone contributes to the promoter activity.	bind
46391	3	11305	5	NULL	NULL	NULL	NULL	statement 1	Process		promotes							activity of		promoter	NULL		NULL	NULL	NULL	NULL	gw60_gene_307_0_87_s_118	12706891	A mutation that disrupted ets binding to the EBS but retained Sp1 binding at this site as well as disruption of both Sp1 and ets binding to the EBS resulted in comparable inhibition of the promoter activity suggesting that at the EBS the binding of ets alone contributes to the promoter activity.	bind
45917	1	11305	6	NULL	NULL	0	NULL	ets	NULL		bind	NULL					NULL			EBS	NULL		NULL	NULL	NULL	NULL	gw60_gene_307_0_87_s_118	12706891	A mutation that disrupted ets binding to the EBS but retained Sp1 binding at this site as well as disruption of both Sp1 and ets binding to the EBS resulted in comparable inhibition of the promoter activity suggesting that at the EBS the binding of ets alone contributes to the promoter activity.	bind
45918	2	11305	6	NULL	NULL	0	NULL	Sp1	NULL		bind	NULL					NULL			EBS	NULL		NULL	NULL	NULL	NULL	gw60_gene_307_0_87_s_118	12706891	A mutation that disrupted ets binding to the EBS but retained Sp1 binding at this site as well as disruption of both Sp1 and ets binding to the EBS resulted in comparable inhibition of the promoter activity suggesting that at the EBS the binding of ets alone contributes to the promoter activity.	bind
45919	3	11305	6	NULL	NULL	0	NULL	statement 1	NULL		contributes to	NULL					NULL	activity of		promoter	NULL		0	NULL	NULL	NULL	gw60_gene_307_0_87_s_118	12706891	A mutation that disrupted ets binding to the EBS but retained Sp1 binding at this site as well as disruption of both Sp1 and ets binding to the EBS resulted in comparable inhibition of the promoter activity suggesting that at the EBS the binding of ets alone contributes to the promoter activity.	bind
45396	1	11306	5	NULL	NULL	NULL	NULL	p53	GP		bind					MDR1	GP			HT site	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_29_27716_s_7	11350951	A mutation that disrupted p53 binding to the MDR1 HT site blocked p53-mediated repression of the  MDR1 promoter in transfection assays.	bind
45397	2	11306	5	NULL	NULL	NULL	NULL	mutation	Process		disrupts					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_29_27716_s_7	11350951	A mutation that disrupted p53 binding to the MDR1 HT site blocked p53-mediated repression of the  MDR1 promoter in transfection assays.	bind
45398	3	11306	5	NULL	NULL	NULL	NULL	p53	GP		mediate					MDR1	GP	repression of		promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_29_27716_s_7	11350951	A mutation that disrupted p53 binding to the MDR1 HT site blocked p53-mediated repression of the  MDR1 promoter in transfection assays.	bind
45399	4	11306	5	NULL	NULL	NULL	NULL	statement 2	Process		block					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_29_27716_s_7	11350951	A mutation that disrupted p53 binding to the MDR1 HT site blocked p53-mediated repression of the  MDR1 promoter in transfection assays.	bind
45920	1	11306	6	NULL	NULL	0	NULL	p53	NULL		bind	NULL				MDR1	NULL			HT site	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_27716_s_7	11350951	A mutation that disrupted p53 binding to the MDR1 HT site blocked p53-mediated repression of the  MDR1 promoter in transfection assays.	bind
45921	2	11306	6	NULL	NULL	0	NULL	p53	NULL		mediates	NULL				MDR1	NULL	repression of		promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_27716_s_7	11350951	A mutation that disrupted p53 binding to the MDR1 HT site blocked p53-mediated repression of the  MDR1 promoter in transfection assays.	bind
51277	3	11306	6	10	NULL	0	NULL	mutation	NULL		disrupt	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_27716_s_7	11350951	A mutation that disrupted p53 binding to the MDR1 HT site blocked p53-mediated repression of the  MDR1 promoter in transfection assays.	bind
51278	4	11306	6	10	NULL	0	NULL	statement 3	NULL		block	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_27716_s_7	11350951	A mutation that disrupted p53 binding to the MDR1 HT site blocked p53-mediated repression of the  MDR1 promoter in transfection assays.	bind
45400	1	11307	5	NULL	NULL	NULL	NULL	NHERF	GP		bind			domain 2		GRK6A	GP	tail			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_34_24328_s_220	10446210	A mutation that reduces the binding of NHERF domain 2 to the GRK6A tail by approximately 4-fold reduces the efficiency with which GRK6A phosphorylates domain 2 by approximately 3-fold.	bind
45401	2	11307	5	NULL	NULL	NULL	NULL	GRK6A	GP		phosphorylate					NHERF	GP		domain 2		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_34_24328_s_220	10446210	A mutation that reduces the binding of NHERF domain 2 to the GRK6A tail by approximately 4-fold reduces the efficiency with which GRK6A phosphorylates domain 2 by approximately 3-fold.	bind
45402	3	11307	5	NULL	NULL	NULL	NULL	mutation	Process		reduces					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_34_24328_s_220	10446210	A mutation that reduces the binding of NHERF domain 2 to the GRK6A tail by approximately 4-fold reduces the efficiency with which GRK6A phosphorylates domain 2 by approximately 3-fold.	bind
45403	4	11307	5	NULL	NULL	NULL	NULL	statement 3	Process		reduces					statement 2	Process	efficiency of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_34_24328_s_220	10446210	A mutation that reduces the binding of NHERF domain 2 to the GRK6A tail by approximately 4-fold reduces the efficiency with which GRK6A phosphorylates domain 2 by approximately 3-fold.	bind
45922	1	11307	6	NULL	NULL	0	NULL	NHERF	NULL		bind	NULL		domain 2		GRK6A 	NULL		tail		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_34_24328_s_220	10446210	A mutation that reduces the binding of NHERF domain 2 to the GRK6A tail by approximately 4-fold reduces the efficiency with which GRK6A phosphorylates domain 2 by approximately 3-fold.	bind
45923	2	11307	6	10	NULL	0	NULL	GRK6A	NULL		phosphorylates	NULL				NHERF	NULL		domain 2		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_34_24328_s_220	10446210	A mutation that reduces the binding of NHERF domain 2 to the GRK6A tail by approximately 4-fold reduces the efficiency with which GRK6A phosphorylates domain 2 by approximately 3-fold.	bind
51279	3	11307	6	10	NULL	0	NULL	mutation 	NULL		reduces	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_34_24328_s_220	10446210	A mutation that reduces the binding of NHERF domain 2 to the GRK6A tail by approximately 4-fold reduces the efficiency with which GRK6A phosphorylates domain 2 by approximately 3-fold.	bind
51280	4	11307	6	10	NULL	0	NULL	statement 3	NULL		reduces	NULL				statement 2	NULL	efficiency of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_34_24328_s_220	10446210	A mutation that reduces the binding of NHERF domain 2 to the GRK6A tail by approximately 4-fold reduces the efficiency with which GRK6A phosphorylates domain 2 by approximately 3-fold.	bind
45404	1	11308	5	NULL	NULL	NULL	NULL	Sp1	GP		bind							proximal		GC box	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_3977_s_62	10330138	A mutation which disrupts both Sp1 and Egr-1 binding to the proximal GC box has been previously described ( 53).	bind
45405	2	11308	5	NULL	NULL	NULL	NULL	Egr-1	GP		bind							proximal		GC box	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_3977_s_62	10330138	A mutation which disrupts both Sp1 and Egr-1 binding to the proximal GC box has been previously described ( 53).	bind
45924	1	11308	6	NULL	NULL	0	NULL	Sp1	NULL		bind	NULL					NULL	proximal		GC box	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_6_3977_s_62	10330138	A mutation which disrupts both Sp1 and Egr-1 binding to the proximal GC box has been previously described ( 53).	bind
45925	2	11308	6	NULL	NULL	0	NULL	Egr-1	NULL		bind	NULL					NULL	proximal		GC-box	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_6_3977_s_62	10330138	A mutation which disrupts both Sp1 and Egr-1 binding to the proximal GC box has been previously described ( 53).	bind
45406	1	11309	5	NULL	NULL	NULL	NULL	CtBP	GP		bind					HPC2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_777_s_381	9858600	A mutation within the 6-aa motif that mediates the binding between CtBP and HPC2 results in a significant but only small decrease in the repressing abilities of HPC2 (Fig.  9).	bind
45926	1	11309	6	NULL	NULL	0	NULL	CtBP	NULL		bind	NULL				HPC2	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_1_777_s_381	9858600	A mutation within the 6-aa motif that mediates the binding between CtBP and HPC2 results in a significant but only small decrease in the repressing abilities of HPC2 (Fig.  9).	bind
45408	1	11310	5	NULL	NULL	NULL	NULL	Sir2	GP		bind					Sir4	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_genesdev_16_12_1528_s_95	12080091	A mutation,  SIR2-H364Y, that disrupts both Sir2 NAD-dependent deacetylase and ADP-ribosyltransferase activities does not prevent binding of Sir2 to Sir4 in vivo (Tanny et al. 1999  ).	bind
45409	2	11310	5	NULL	NULL	NULL	NULL	SIR2	GP	mutant	disrupts			H364Y		Sir2 NAD-dependent deacetylase 	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_12_1528_s_95	12080091	A mutation,  SIR2-H364Y, that disrupts both Sir2 NAD-dependent deacetylase and ADP-ribosyltransferase activities does not prevent binding of Sir2 to Sir4 in vivo (Tanny et al. 1999  ).	bind
45410	3	11310	5	NULL	NULL	NULL	NULL	SIR2	GP	mutant	disrupts			H364Y		ADP-ribosyltransferase 	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_16_12_1528_s_95	12080091	A mutation,  SIR2-H364Y, that disrupts both Sir2 NAD-dependent deacetylase and ADP-ribosyltransferase activities does not prevent binding of Sir2 to Sir4 in vivo (Tanny et al. 1999  ).	bind
68150	4	11310	5	NULL	NULL	0	NULL	SIR2	GP	mutant	does not prevent			H364Y		statement 1	Process				NULL	in vivo	0	NULL	NULL	NULL	gw60_genesdev_16_12_1528_s_95	12080091	A mutation,  SIR2-H364Y, that disrupts both Sir2 NAD-dependent deacetylase and ADP-ribosyltransferase activities does not prevent binding of Sir2 to Sir4 in vivo (Tanny et al. 1999  ).	bind
45927	1	11310	6	NULL	NULL	0	NULL	Sir2	NULL		bind	NULL				Sir4	NULL				NULL	in vivo	0	NULL	NULL	NULL	gw60_genesdev_16_12_1528_s_95	12080091	A mutation,  SIR2-H364Y, that disrupts both Sir2 NAD-dependent deacetylase and ADP-ribosyltransferase activities does not prevent binding of Sir2 to Sir4 in vivo (Tanny et al. 1999  ).	bind
45928	2	11310	6	NULL	NULL	0	NULL	SIR2	NULL	mutant	disrupts	NULL		H364Y		Sir2 NAD-dependent deacetylase	NULL	activity of			NULL		0	NULL	NULL	NULL	gw60_genesdev_16_12_1528_s_95	12080091	A mutation,  SIR2-H364Y, that disrupts both Sir2 NAD-dependent deacetylase and ADP-ribosyltransferase activities does not prevent binding of Sir2 to Sir4 in vivo (Tanny et al. 1999  ).	bind
45929	3	11310	6	NULL	NULL	0	NULL	SIR2	NULL	mutant	disrupts	NULL		H364Y		ADP-ribosyltransferase	NULL	activity of			NULL		0	NULL	NULL	NULL	gw60_genesdev_16_12_1528_s_95	12080091	A mutation,  SIR2-H364Y, that disrupts both Sir2 NAD-dependent deacetylase and ADP-ribosyltransferase activities does not prevent binding of Sir2 to Sir4 in vivo (Tanny et al. 1999  ).	bind
45930	4	11310	6	10	NULL	0	NULL	SIR2		mutant	does not prevent			H364Y		statement 1					NULL	in vivo	NULL	NULL	NULL	NULL	gw60_genesdev_16_12_1528_s_95	12080091	A mutation,  SIR2-H364Y, that disrupts both Sir2 NAD-dependent deacetylase and ADP-ribosyltransferase activities does not prevent binding of Sir2 to Sir4 in vivo (Tanny et al. 1999  ).	bind
45412	1	11311	5	NULL	NULL	NULL	NULL	CREB	GP		bind									CRE	NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_55_6_1094_s_174	10347253	A mutational analysis (German and Wang, 1994  ; Eggers et al., 1998  ) and the overexpression of a dominant-negative CREB mutant (Eggers et al., 1998  ) have shown that the activation by cAMP of this promoter is mediated by CREB binding to the CRE.	bind
45931	1	11311	6	NULL	NULL	0	NULL	CREB	NULL		bind	NULL					NULL			CRE	NULL		0	NULL	NULL	NULL	gw60_molpharmacol_55_6_1094_s_174	10347253	A mutational analysis (German and Wang, 1994  ; Eggers et al., 1998  ) and the overexpression of a dominant-negative CREB mutant (Eggers et al., 1998  ) have shown that the activation by cAMP of this promoter is mediated by CREB binding to the CRE.	bind
45413	1	11312	5	NULL	NULL	NULL	NULL			single mutation of	reduces		significantly	D313A		eIF5A	GP	binding of	Lys		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_27_28697_s_315	15100216	A mutational analysis of residues forming the NAD and spermidine binding sites revealed a single mutation (D313A) that significantly reduced eIF5A(Lys) binding ( ).	bind
45932	1	11312	6	10	NULL	0	NULL		NULL	mutant	reduces	NULL	significantly	D313A		eIF5A	NULL	binding of	Lys		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_27_28697_s_315	15100216	A mutational analysis of residues forming the NAD and spermidine binding sites revealed a single mutation (D313A) that significantly reduced eIF5A(Lys) binding ( ).	bind
45414	1	11314	5	NULL	NULL	NULL	NULL	enterotoxin B	GP	staphylococcal	bind					T cell receptor	GP		beta chain		NULL		NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_55_0_77_s_792	11544350	A mutational analysis of the binding of staphylococcal enterotoxins  B and C3 to the T cell receptor beta chain and major histocompatibility complex class  II.	bind
45415	2	11314	5	NULL	NULL	NULL	NULL	enterotoxin B	GP	staphylococcal	bind					major histocompatibility complex class II	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_55_0_77_s_792	11544350	A mutational analysis of the binding of staphylococcal enterotoxins  B and C3 to the T cell receptor beta chain and major histocompatibility complex class  II.	bind
45416	3	11314	5	NULL	NULL	NULL	NULL	enterotoxin C3	GP	staphylococcal	bind					T cell receptor	GP		beta chain		NULL		NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_55_0_77_s_792	11544350	A mutational analysis of the binding of staphylococcal enterotoxins  B and C3 to the T cell receptor beta chain and major histocompatibility complex class  II.	bind
45417	4	11314	5	NULL	NULL	NULL	NULL	enterotoxin C3	GP	staphylococcal	bind					major histocompatibility complex class II	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_55_0_77_s_792	11544350	A mutational analysis of the binding of staphylococcal enterotoxins  B and C3 to the T cell receptor beta chain and major histocompatibility complex class  II.	bind
45933	1	11314	6	NULL	NULL	0	NULL	enterotoxin B	NULL	Staphylococcal	bind	NULL				T cell receptor 	NULL		beta chain		NULL		NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_55_0_77_s_792	11544350	A mutational analysis of the binding of staphylococcal enterotoxins  B and C3 to the T cell receptor beta chain and major histocompatibility complex class  II.	bind
45934	2	11314	6	NULL	NULL	0	NULL	enterotoxin C3	NULL	Staphylococcal	bind	NULL				major histocompatibility complex class II	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_55_0_77_s_792	11544350	A mutational analysis of the binding of staphylococcal enterotoxins  B and C3 to the T cell receptor beta chain and major histocompatibility complex class  II.	bind
51459	3	11314	6	10	NULL	0	NULL	enterotoxins B	NULL	staphylococcal 	bind	NULL				major histocompatibility complex class II	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_55_0_77_s_792	11544350	A mutational analysis of the binding of staphylococcal enterotoxins  B and C3 to the T cell receptor beta chain and major histocompatibility complex class  II.	bind
51460	4	11314	6	10	NULL	0	NULL	enterotoxins C3	NULL	staphylococcal	bind	NULL				T cell receptor	NULL		beta chain		NULL		NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_55_0_77_s_792	11544350	A mutational analysis of the binding of staphylococcal enterotoxins  B and C3 to the T cell receptor beta chain and major histocompatibility complex class  II.	bind
45418	1	11316	5	NULL	NULL	NULL	NULL	Ras	GP		bind					Raf	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_30363_s_35	10887184	A mutational analysis of the RBD binding site showed that Gln66, Lys84, and Arg89 are the major contributors to the binding affinity between Ras and Raf ( 1).	bind
45419	2	11316	5	NULL	NULL	NULL	NULL				contribute to		major	Gln66 in RBD binding site		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_30363_s_35	10887184	A mutational analysis of the RBD binding site showed that Gln66, Lys84, and Arg89 are the major contributors to the binding affinity between Ras and Raf ( 1).	bind
45420	3	11316	5	NULL	NULL	NULL	NULL				contribute to		major	Lys84 in RBD binding site		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_30363_s_35	10887184	A mutational analysis of the RBD binding site showed that Gln66, Lys84, and Arg89 are the major contributors to the binding affinity between Ras and Raf ( 1).	bind
45421	4	11316	5	NULL	NULL	NULL	NULL				contribute to		major	Arg89 in RBD binding site		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_30363_s_35	10887184	A mutational analysis of the RBD binding site showed that Gln66, Lys84, and Arg89 are the major contributors to the binding affinity between Ras and Raf ( 1).	bind
45937	1	11316	6	NULL	NULL	0	NULL	Ras	NULL		bind	NULL				Raf	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_39_30363_s_35	10887184	A mutational analysis of the RBD binding site showed that Gln66, Lys84, and Arg89 are the major contributors to the binding affinity between Ras and Raf ( 1).	bind
45938	2	11316	6	NULL	NULL	0	NULL		NULL		contributes to	NULL		RBD binding site;; Gln66		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_39_30363_s_35	10887184	A mutational analysis of the RBD binding site showed that Gln66, Lys84, and Arg89 are the major contributors to the binding affinity between Ras and Raf ( 1).	bind
45939	3	11316	6	NULL	NULL	0	NULL		NULL		contributes to	NULL		RBD binding site;; Lys84		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_39_30363_s_35	10887184	A mutational analysis of the RBD binding site showed that Gln66, Lys84, and Arg89 are the major contributors to the binding affinity between Ras and Raf ( 1).	bind
45940	4	11316	6	NULL	NULL	0	NULL		NULL		contributes to	NULL		RBD binding site;; Arg89		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_39_30363_s_35	10887184	A mutational analysis of the RBD binding site showed that Gln66, Lys84, and Arg89 are the major contributors to the binding affinity between Ras and Raf ( 1).	bind
45422	1	11320	5	NULL	NULL	NULL	NULL	Cdc42p	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_23	10066831	A myriad of Cdc42p downstream effectors interact with the activated (GTP-bound) form of Cdc42p, thereby inducing a number of downstream events, including rearrangements of the actin cytoskeletal network and protein kinase-dependent induction of transcription, which are increasingly coming into view.	bind
45423	2	11320	5	NULL	NULL	NULL	NULL	Cdc42p downstream effectors	GP		interact with					statement 1	Process	activated			NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_23	10066831	A myriad of Cdc42p downstream effectors interact with the activated (GTP-bound) form of Cdc42p, thereby inducing a number of downstream events, including rearrangements of the actin cytoskeletal network and protein kinase-dependent induction of transcription, which are increasingly coming into view.	bind
45424	3	11320	5	NULL	NULL	NULL	NULL	statement 2	Process		induce					downstream events	Process				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_23	10066831	A myriad of Cdc42p downstream effectors interact with the activated (GTP-bound) form of Cdc42p, thereby inducing a number of downstream events, including rearrangements of the actin cytoskeletal network and protein kinase-dependent induction of transcription, which are increasingly coming into view.	bind
45425	4	11320	5	NULL	NULL	NULL	NULL	downstream events	Process		include					actin cytoskeletal network	CellComponent	rearrangements of			NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_23	10066831	A myriad of Cdc42p downstream effectors interact with the activated (GTP-bound) form of Cdc42p, thereby inducing a number of downstream events, including rearrangements of the actin cytoskeletal network and protein kinase-dependent induction of transcription, which are increasingly coming into view.	bind
45426	5	11320	5	NULL	NULL	NULL	NULL	transcription	Process	induction of	is dependent on					protein kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_23	10066831	A myriad of Cdc42p downstream effectors interact with the activated (GTP-bound) form of Cdc42p, thereby inducing a number of downstream events, including rearrangements of the actin cytoskeletal network and protein kinase-dependent induction of transcription, which are increasingly coming into view.	bind
45427	6	11320	5	NULL	NULL	NULL	NULL	downstream events	Process		include					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_23	10066831	A myriad of Cdc42p downstream effectors interact with the activated (GTP-bound) form of Cdc42p, thereby inducing a number of downstream events, including rearrangements of the actin cytoskeletal network and protein kinase-dependent induction of transcription, which are increasingly coming into view.	bind
46093	1	11320	6	10	NULL	0	NULL	GTP	NULL		bind	NULL				Cdc42p	NULL				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_23	10066831	A myriad of Cdc42p downstream effectors interact with the activated (GTP-bound) form of Cdc42p, thereby inducing a number of downstream events, including rearrangements of the actin cytoskeletal network and protein kinase-dependent induction of transcription, which are increasingly coming into view.	bind
46094	2	11320	6	10	NULL	0	NULL	Cdc42p downstream effectors	NULL		interacts with	NULL				statement 1	NULL	activated			NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_23	10066831	A myriad of Cdc42p downstream effectors interact with the activated (GTP-bound) form of Cdc42p, thereby inducing a number of downstream events, including rearrangements of the actin cytoskeletal network and protein kinase-dependent induction of transcription, which are increasingly coming into view.	bind
46095	3	11320	6	NULL	NULL	0	NULL	statement 2	NULL		includes	NULL				actin cytoskeleton network	NULL	rearrangements of 			NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_23	10066831	A myriad of Cdc42p downstream effectors interact with the activated (GTP-bound) form of Cdc42p, thereby inducing a number of downstream events, including rearrangements of the actin cytoskeletal network and protein kinase-dependent induction of transcription, which are increasingly coming into view.	bind
46096	4	11320	6	NULL	NULL	0	NULL	transcription	NULL	induction of	is dependent on	NULL				protein kinase	NULL				NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_23	10066831	A myriad of Cdc42p downstream effectors interact with the activated (GTP-bound) form of Cdc42p, thereby inducing a number of downstream events, including rearrangements of the actin cytoskeletal network and protein kinase-dependent induction of transcription, which are increasingly coming into view.	bind
46098	5	11320	6	NULL	NULL	0	NULL	statement 2	NULL		induces	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_54_s_23	10066831	A myriad of Cdc42p downstream effectors interact with the activated (GTP-bound) form of Cdc42p, thereby inducing a number of downstream events, including rearrangements of the actin cytoskeletal network and protein kinase-dependent induction of transcription, which are increasingly coming into view.	bind
45428	1	11321	5	NULL	NULL	NULL	NULL	MC	GP		bind					MRD	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_3_926_s_28	11158572	A mystery has remained regarding the NADH requirement for binding of MC to MRD, because this cofactor would only be expected for the flavoreductase-mediated bioactivation of MC.	bind
45429	2	11321	5	NULL	NULL	NULL	NULL	flavoreductase	GP		mediates					MC	GP	bioactivation of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_3_926_s_28	11158572	A mystery has remained regarding the NADH requirement for binding of MC to MRD, because this cofactor would only be expected for the flavoreductase-mediated bioactivation of MC.	bind
45430	3	11321	5	NULL	NULL	NULL	NULL	NADH	Chemical		is required for		potentially			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_3_926_s_28	11158572	A mystery has remained regarding the NADH requirement for binding of MC to MRD, because this cofactor would only be expected for the flavoreductase-mediated bioactivation of MC.	bind
45941	1	11321	6	NULL	NULL	0	NULL	MC	NULL		bind	NULL				MRD	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_98_3_926_s_28	11158572	A mystery has remained regarding the NADH requirement for binding of MC to MRD, because this cofactor would only be expected for the flavoreductase-mediated bioactivation of MC.	bind
45431	1	11322	5	NULL	NULL	NULL	NULL	Hrd3p	GP	truncated	bind			N-terminal		Hrd1p	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_9_1827_s_214	16619026	A N-terminally  truncated form of Hrd3p still binds to Hrd1p and maintains it at wild-type levels,  although the function of the Hrd1p ligase complex is abolished (  et al and data not shown).	bind
45432	2	11322	5	NULL	NULL	NULL	NULL	Hrd3p	GP	truncated	abolishes			N-terminal		Hrd1p ligase complex	GP	function of			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_9_1827_s_214	16619026	A N-terminally  truncated form of Hrd3p still binds to Hrd1p and maintains it at wild-type levels,  although the function of the Hrd1p ligase complex is abolished (  et al and data not shown).	bind
45942	1	11322	6	NULL	NULL	0	NULL	Hrd3p	NULL	deletion of	bind	NULL		N-terminal		Hrd1p	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_25_9_1827_s_214	16619026	A N-terminally  truncated form of Hrd3p still binds to Hrd1p and maintains it at wild-type levels,  although the function of the Hrd1p ligase complex is abolished (  et al and data not shown).	bind
51461	2	11322	6	10	NULL	0	NULL	Hrd3p	NULL	deletion of	abolishes	NULL		N-terminal		Hrd1p ligase complex	NULL	function of			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_9_1827_s_214	16619026	A N-terminally  truncated form of Hrd3p still binds to Hrd1p and maintains it at wild-type levels,  although the function of the Hrd1p ligase complex is abolished (  et al and data not shown).	bind
45433	1	11323	5	NULL	NULL	NULL	NULL	ACh	Chemical		is					acetylcholine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neuron_16_5_905_s_4	8630247	A nAChR normally binds acetylcholine (ACh) and undergoes a conformational change that opens a cation-selective channel for several milliseconds.	bind
45434	2	11323	5	NULL	NULL	NULL	NULL	nAChR	GP		bind					ACh	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_neuron_16_5_905_s_4	8630247	A nAChR normally binds acetylcholine (ACh) and undergoes a conformational change that opens a cation-selective channel for several milliseconds.	bind
45435	3	11323	5	NULL	NULL	NULL	NULL	nAChR	GP		undergoes					conformational change	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_16_5_905_s_4	8630247	A nAChR normally binds acetylcholine (ACh) and undergoes a conformational change that opens a cation-selective channel for several milliseconds.	bind
45436	4	11323	5	NULL	NULL	NULL	NULL	statement 2	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_neuron_16_5_905_s_4	8630247	A nAChR normally binds acetylcholine (ACh) and undergoes a conformational change that opens a cation-selective channel for several milliseconds.	bind
45437	5	11323	5	NULL	NULL	NULL	NULL	statement 3	Process		open					cation-selective channel	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_16_5_905_s_4	8630247	A nAChR normally binds acetylcholine (ACh) and undergoes a conformational change that opens a cation-selective channel for several milliseconds.	bind
45943	1	11323	6	NULL	NULL	0	NULL	nAChR	NULL		bind	NULL				ACh	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_16_5_905_s_4	8630247	A nAChR normally binds acetylcholine (ACh) and undergoes a conformational change that opens a cation-selective channel for several milliseconds.	bind
45944	2	11323	6	NULL	NULL	0	NULL	ACh	NULL		is	NULL				acetylcholine	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_16_5_905_s_4	8630247	A nAChR normally binds acetylcholine (ACh) and undergoes a conformational change that opens a cation-selective channel for several milliseconds.	bind
45945	3	11323	6	NULL	NULL	0	NULL	nAChR	NULL		undergoes a	NULL				conformational change	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_16_5_905_s_4	8630247	A nAChR normally binds acetylcholine (ACh) and undergoes a conformational change that opens a cation-selective channel for several milliseconds.	bind
45946	4	11323	6	10	NULL	0	NULL	statement 3	NULL		opens a	NULL				cation-selective channel	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuron_16_5_905_s_4	8630247	A nAChR normally binds acetylcholine (ACh) and undergoes a conformational change that opens a cation-selective channel for several milliseconds.	bind
51462	5	11323	6	10	NULL	0	NULL	statement 3	NULL		leads to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_16_5_905_s_4	8630247	A nAChR normally binds acetylcholine (ACh) and undergoes a conformational change that opens a cation-selective channel for several milliseconds.	bind
45438	1	11324	5	NULL	NULL	NULL	NULL	Spt5p	GP		bind			NGN - KOW region		Spt4p	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_17_3643_s_105	12202748	A natural corollary to the finding that an NGN - KOW region of Spt5p binds Spt4p is that their archaeal homologues, rpoE"` and NusG, may also associate.	bind
45439	2	11324	5	NULL	NULL	NULL	NULL	rpoE"	GP	archaeal	is a homolog of					Spt5p	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_17_3643_s_105	12202748	A natural corollary to the finding that an NGN - KOW region of Spt5p binds Spt4p is that their archaeal homologues, rpoE"` and NusG, may also associate.	bind
45440	3	11324	5	NULL	NULL	NULL	NULL	NusG	GP	archaeal	is a homolog of					Spt4p	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_17_3643_s_105	12202748	A natural corollary to the finding that an NGN - KOW region of Spt5p binds Spt4p is that their archaeal homologues, rpoE"` and NusG, may also associate.	bind
45441	4	11324	5	NULL	NULL	NULL	NULL	statement 2	Process		associate with		may			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_17_3643_s_105	12202748	A natural corollary to the finding that an NGN - KOW region of Spt5p binds Spt4p is that their archaeal homologues, rpoE"` and NusG, may also associate.	bind
45947	1	11324	6	NULL	NULL	0	NULL	Spt5p	NULL		bind	NULL		NGN - KOW region		Spt4p	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_17_3643_s_105	12202748	A natural corollary to the finding that an NGN - KOW region of Spt5p binds Spt4p is that their archaeal homologues, rpoE"` and NusG, may also associate.	bind
45948	2	11324	6	NULL	NULL	0	NULL	rpoE''	NULL	archaeal	is homologous to	NULL				Spt5p	NULL				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_17_3643_s_105	12202748	A natural corollary to the finding that an NGN - KOW region of Spt5p binds Spt4p is that their archaeal homologues, rpoE"` and NusG, may also associate.	bind
52956	3	11324	6	NULL	NULL	0	NULL	NusG	NULL	archaeal	is homologous to	NULL				Spt5p	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_17_3643_s_105	12202748	A natural corollary to the finding that an NGN - KOW region of Spt5p binds Spt4p is that their archaeal homologues, rpoE"` and NusG, may also associate.	bind
52957	4	11324	6	10	NULL	0	NULL	statement 2			associates with		may			statement 3					NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_17_3643_s_105	12202748	A natural corollary to the finding that an NGN - KOW region of Spt5p binds Spt4p is that their archaeal homologues, rpoE"` and NusG, may also associate.	bind
45442	1	11325	5	NULL	NULL	NULL	NULL	cysteine protease virulence factor	GP	natural variant of;; group A Streptococcus	bind		preferentially	RGD motif		alphaV beta3	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_15_4461_s_442	12867455	A natural variant of the cysteine protease virulence factor of group A  Streptococcus with an arginine-glycine-aspartic acid (RGD) motif preferentially binds human integrins  alphaV beta3 and  alphaIIb beta3.	bind
45443	2	11325	5	NULL	NULL	NULL	NULL	alphaV beta3	GP		is a type of					integrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_15_4461_s_442	12867455	A natural variant of the cysteine protease virulence factor of group A  Streptococcus with an arginine-glycine-aspartic acid (RGD) motif preferentially binds human integrins  alphaV beta3 and  alphaIIb beta3.	bind
45444	3	11325	5	NULL	NULL	NULL	NULL	RGD motif	AminoAcid		is					arginine-glycine-aspartic acid motif 	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_15_4461_s_442	12867455	A natural variant of the cysteine protease virulence factor of group A  Streptococcus with an arginine-glycine-aspartic acid (RGD) motif preferentially binds human integrins  alphaV beta3 and  alphaIIb beta3.	bind
45445	4	11325	5	NULL	NULL	NULL	NULL	cysteine protease virulence factor	GP	natural variant of;; group A Streptococcus	bind		preferentially	RGD motif		alphaIIb beta3	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_15_4461_s_442	12867455	A natural variant of the cysteine protease virulence factor of group A  Streptococcus with an arginine-glycine-aspartic acid (RGD) motif preferentially binds human integrins  alphaV beta3 and  alphaIIb beta3.	bind
45446	5	11325	5	NULL	NULL	NULL	NULL	alphaIIb beta3	AminoAcid		is a type of					integrin	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_15_4461_s_442	12867455	A natural variant of the cysteine protease virulence factor of group A  Streptococcus with an arginine-glycine-aspartic acid (RGD) motif preferentially binds human integrins  alphaV beta3 and  alphaIIb beta3.	bind
45949	1	11325	6	10	NULL	0	NULL	cysteine protease virulence factor 		natural variant of;;group A Streptococcus	bind		preferentially	RGD motif		alphaV beta3		human			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_15_4461_s_442	12867455	A natural variant of the cysteine protease virulence factor of group A  Streptococcus with an arginine-glycine-aspartic acid (RGD) motif preferentially binds human integrins  alphaV beta3 and  alphaIIb beta3.	bind
45950	2	11325	6	10	NULL	0	NULL	cysteine protease virulence factor		natural variant of;;group A Streptococcus	bind		preferentially	RGD motif		alphaIIb beta3		human			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_15_4461_s_442	12867455	A natural variant of the cysteine protease virulence factor of group A  Streptococcus with an arginine-glycine-aspartic acid (RGD) motif preferentially binds human integrins  alphaV beta3 and  alphaIIb beta3.	bind
45951	3	11325	6	NULL	NULL	0	NULL	RGD	NULL		is	NULL				arginine-glycine-aspartic acid	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_185_15_4461_s_442	12867455	A natural variant of the cysteine protease virulence factor of group A  Streptococcus with an arginine-glycine-aspartic acid (RGD) motif preferentially binds human integrins  alphaV beta3 and  alphaIIb beta3.	bind
51463	4	11325	6	10	NULL	0	NULL	alphaV beta3	NULL		is a type of	NULL				integrin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_185_15_4461_s_442	12867455	A natural variant of the cysteine protease virulence factor of group A  Streptococcus with an arginine-glycine-aspartic acid (RGD) motif preferentially binds human integrins  alphaV beta3 and  alphaIIb beta3.	bind
51464	5	11325	6	10	NULL	0	NULL	alphaIIb beta3	NULL		is a type of	NULL				integrin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_185_15_4461_s_442	12867455	A natural variant of the cysteine protease virulence factor of group A  Streptococcus with an arginine-glycine-aspartic acid (RGD) motif preferentially binds human integrins  alphaV beta3 and  alphaIIb beta3.	bind
45447	1	11331	5	NULL	NULL	NULL	NULL	PR39	GP		is a type of					naturally occurring antibacterial peptide	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_9_877_s_153	11348996	A naturally occurring antibacterial peptide, PR39, which reversibly binds the 26S proteasome and blocks the degradation of IkappaBalpha by the ubiquitin-preoteasome pathway, suppresses VCAM-1 and ICAM-1 gene expression in TNF-alpha - activated human ECs and reduces the size of myocardial infarction in an in vivo mouse model of coronary ligature.	bind
45448	2	11331	5	NULL	NULL	NULL	NULL	PR39	GP		bind		reversibly			26S proteasome	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_9_877_s_153	11348996	A naturally occurring antibacterial peptide, PR39, which reversibly binds the 26S proteasome and blocks the degradation of IkappaBalpha by the ubiquitin-preoteasome pathway, suppresses VCAM-1 and ICAM-1 gene expression in TNF-alpha - activated human ECs and reduces the size of myocardial infarction in an in vivo mouse model of coronary ligature.	bind
45449	3	11331	5	NULL	NULL	NULL	NULL	statement 2	Process		block					IkappaBalpha	GP	degradation of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_9_877_s_153	11348996	A naturally occurring antibacterial peptide, PR39, which reversibly binds the 26S proteasome and blocks the degradation of IkappaBalpha by the ubiquitin-preoteasome pathway, suppresses VCAM-1 and ICAM-1 gene expression in TNF-alpha - activated human ECs and reduces the size of myocardial infarction in an in vivo mouse model of coronary ligature.	bind
45450	4	11331	5	NULL	NULL	NULL	NULL	statement 3	Process		occurs by					ubiquitin-preoteasome pathway	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_88_9_877_s_153	11348996	A naturally occurring antibacterial peptide, PR39, which reversibly binds the 26S proteasome and blocks the degradation of IkappaBalpha by the ubiquitin-preoteasome pathway, suppresses VCAM-1 and ICAM-1 gene expression in TNF-alpha - activated human ECs and reduces the size of myocardial infarction in an in vivo mouse model of coronary ligature.	bind
45451	5	11331	5	NULL	NULL	NULL	NULL	PR39	GP		supress					VCAM-1 gene	GP	expression of			NULL	TNF-alpha - activated human ECs	NULL	NULL	NULL	NULL	gw60_circulationres_88_9_877_s_153	11348996	A naturally occurring antibacterial peptide, PR39, which reversibly binds the 26S proteasome and blocks the degradation of IkappaBalpha by the ubiquitin-preoteasome pathway, suppresses VCAM-1 and ICAM-1 gene expression in TNF-alpha - activated human ECs and reduces the size of myocardial infarction in an in vivo mouse model of coronary ligature.	bind
45452	6	11331	5	NULL	NULL	NULL	NULL	PR39	GP		supress					ICAM-1 gene	GP	expression of			NULL	TNF-alpha - activated human ECs	NULL	NULL	NULL	NULL	gw60_circulationres_88_9_877_s_153	11348996	A naturally occurring antibacterial peptide, PR39, which reversibly binds the 26S proteasome and blocks the degradation of IkappaBalpha by the ubiquitin-preoteasome pathway, suppresses VCAM-1 and ICAM-1 gene expression in TNF-alpha - activated human ECs and reduces the size of myocardial infarction in an in vivo mouse model of coronary ligature.	bind
45453	7	11331	5	NULL	NULL	NULL	NULL	PR39	GP		reduces					myocardial infarction	MedicalFinding	size of			NULL	in vivo mouse model of coronary ligature	NULL	NULL	NULL	NULL	gw60_circulationres_88_9_877_s_153	11348996	A naturally occurring antibacterial peptide, PR39, which reversibly binds the 26S proteasome and blocks the degradation of IkappaBalpha by the ubiquitin-preoteasome pathway, suppresses VCAM-1 and ICAM-1 gene expression in TNF-alpha - activated human ECs and reduces the size of myocardial infarction in an in vivo mouse model of coronary ligature.	bind
45952	1	11331	6	NULL	NULL	0	NULL	PR39	NULL		is a type of	NULL				antibacterial peptide	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_88_9_877_s_153	11348996	A naturally occurring antibacterial peptide, PR39, which reversibly binds the 26S proteasome and blocks the degradation of IkappaBalpha by the ubiquitin-preoteasome pathway, suppresses VCAM-1 and ICAM-1 gene expression in TNF-alpha - activated human ECs and reduces the size of myocardial infarction in an in vivo mouse model of coronary ligature.	bind
45953	2	11331	6	NULL	NULL	0	NULL	PR39	NULL		bind	NULL	reversibly			26S proteasome	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_88_9_877_s_153	11348996	A naturally occurring antibacterial peptide, PR39, which reversibly binds the 26S proteasome and blocks the degradation of IkappaBalpha by the ubiquitin-preoteasome pathway, suppresses VCAM-1 and ICAM-1 gene expression in TNF-alpha - activated human ECs and reduces the size of myocardial infarction in an in vivo mouse model of coronary ligature.	bind
45954	3	11331	6	NULL	NULL	0	NULL	ubiquitin-preoteasome pathway	NULL		degrades	NULL				IkappaBalpha	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_88_9_877_s_153	11348996	A naturally occurring antibacterial peptide, PR39, which reversibly binds the 26S proteasome and blocks the degradation of IkappaBalpha by the ubiquitin-preoteasome pathway, suppresses VCAM-1 and ICAM-1 gene expression in TNF-alpha - activated human ECs and reduces the size of myocardial infarction in an in vivo mouse model of coronary ligature.	bind
45955	4	11331	6	NULL	NULL	0	NULL	statement 2	NULL		blocks	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_88_9_877_s_153	11348996	A naturally occurring antibacterial peptide, PR39, which reversibly binds the 26S proteasome and blocks the degradation of IkappaBalpha by the ubiquitin-preoteasome pathway, suppresses VCAM-1 and ICAM-1 gene expression in TNF-alpha - activated human ECs and reduces the size of myocardial infarction in an in vivo mouse model of coronary ligature.	bind
45958	5	11331	6	NULL	NULL	0	NULL	statement 2	NULL		suppresses	NULL				VCAM-1 gene	NULL	expression of			NULL	TNF-alpha - activated human ECs	0	NULL	NULL	NULL	gw60_circulationres_88_9_877_s_153	11348996	A naturally occurring antibacterial peptide, PR39, which reversibly binds the 26S proteasome and blocks the degradation of IkappaBalpha by the ubiquitin-preoteasome pathway, suppresses VCAM-1 and ICAM-1 gene expression in TNF-alpha - activated human ECs and reduces the size of myocardial infarction in an in vivo mouse model of coronary ligature.	bind
45959	6	11331	6	NULL	NULL	0	NULL	statement 2	NULL		suppresses	NULL				ICAM-1 gene	NULL	expression of			NULL	TNF-alpha - activated human ECs	NULL	NULL	NULL	NULL	gw60_circulationres_88_9_877_s_153	11348996	A naturally occurring antibacterial peptide, PR39, which reversibly binds the 26S proteasome and blocks the degradation of IkappaBalpha by the ubiquitin-preoteasome pathway, suppresses VCAM-1 and ICAM-1 gene expression in TNF-alpha - activated human ECs and reduces the size of myocardial infarction in an in vivo mouse model of coronary ligature.	bind
45960	7	11331	6	NULL	NULL	0	NULL	statement 2	NULL		reduces	NULL				myocardial infarction	NULL	size of			NULL	in vivo mouse model of coronary ligature	0	NULL	NULL	NULL	gw60_circulationres_88_9_877_s_153	11348996	A naturally occurring antibacterial peptide, PR39, which reversibly binds the 26S proteasome and blocks the degradation of IkappaBalpha by the ubiquitin-preoteasome pathway, suppresses VCAM-1 and ICAM-1 gene expression in TNF-alpha - activated human ECs and reduces the size of myocardial infarction in an in vivo mouse model of coronary ligature.	bind
45454	1	11332	5	NULL	NULL	NULL	NULL	parafibromin	GP	mutant	does not bind					PAF1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_5052_s_172	15923622	A naturally occurring loss-of-function mutant of parafibromin lacks PAF1 and RNAP  II binding activity.	bind
45455	2	11332	5	NULL	NULL	NULL	NULL	parafibromin	GP	mutant	does not bind					RNAP II	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_5052_s_172	15923622	A naturally occurring loss-of-function mutant of parafibromin lacks PAF1 and RNAP  II binding activity.	bind
45961	1	11332	6	NULL	NULL	0	NULL	parafibromin	NULL	mutant	does not bind	NULL				PAF1	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_12_5052_s_172	15923622	A naturally occurring loss-of-function mutant of parafibromin lacks PAF1 and RNAP  II binding activity.	bind
45962	2	11332	6	NULL	NULL	0	NULL	parafibromin	NULL	mutant	does not bind	NULL				RNAP II	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_12_5052_s_172	15923622	A naturally occurring loss-of-function mutant of parafibromin lacks PAF1 and RNAP  II binding activity.	bind
45456	1	11333	5	NULL	NULL	NULL	NULL	Fc gamma RIIA	GP		is mutated to			Q127		Fc gamma RIIA	GP		K127		NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_3_1252_s_408	10678934	A naturally occurring mutation in Fc gamma RIIA: a Q to K127 change confers unique IgG binding properties to the R131 allelic form of the receptor.	bind
45458	3	11333	5	NULL	NULL	NULL	NULL	R131	GP		is an allelic form of					Fc gamma RIIA	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_3_1252_s_408	10678934	A naturally occurring mutation in Fc gamma RIIA: a Q to K127 change confers unique IgG binding properties to the R131 allelic form of the receptor.	bind
45459	2	11333	5	NULL	NULL	NULL	NULL	R131	GP		bind		uniquely			IgG	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_3_1252_s_408	10678934	A naturally occurring mutation in Fc gamma RIIA: a Q to K127 change confers unique IgG binding properties to the R131 allelic form of the receptor.	bind
45460	4	11333	5	NULL	NULL	NULL	NULL	statement 1	Process		confers					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_3_1252_s_408	10678934	A naturally occurring mutation in Fc gamma RIIA: a Q to K127 change confers unique IgG binding properties to the R131 allelic form of the receptor.	bind
46104	1	11333	6	10	NULL	0	NULL	Fc gamma RIIA	NULL		is changed to	NULL		Q127		Fc gamma RIIA	NULL		K127		NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_3_1252_s_408	10678934	A naturally occurring mutation in Fc gamma RIIA: a Q to K127 change confers unique IgG binding properties to the R131 allelic form of the receptor.	bind
46105	2	11333	6	10	NULL	0	NULL	IgG			bind		uniquely			R131					NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_3_1252_s_408	10678934	A naturally occurring mutation in Fc gamma RIIA: a Q to K127 change confers unique IgG binding properties to the R131 allelic form of the receptor.	bind
46106	4	11333	6	10	NULL	0	NULL	statement 1			confers					statement 2					NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_3_1252_s_408	10678934	A naturally occurring mutation in Fc gamma RIIA: a Q to K127 change confers unique IgG binding properties to the R131 allelic form of the receptor.	bind
60571	3	11333	6	10	NULL	0	NULL	R131			is an allelic form of					Fc gamma RIIA					NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_3_1252_s_408	10678934	A naturally occurring mutation in Fc gamma RIIA: a Q to K127 change confers unique IgG binding properties to the R131 allelic form of the receptor.	bind
45461	1	11334	5	NULL	NULL	NULL	NULL	EC-SOD	GP		is substituted with			ECM-binding region;;Arg213		EC-SOD	GP		ECM-binding region;;Gly		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_21_22152_s_31	15044467	A naturally occurring mutation in the ECM-binding region of EC-SOD substitutes Arg213 for Gly ( Fig. 1) (  -  ).	bind
45963	1	11334	6	NULL	NULL	0	NULL	EC-SOD	NULL	mutant	is substituted with	NULL		ECM-binding region;; Arg213		EC-SOD	NULL	mutant	ECM-binding region;; Gly		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_21_22152_s_31	15044467	A naturally occurring mutation in the ECM-binding region of EC-SOD substitutes Arg213 for Gly ( Fig. 1) (  -  ).	bind
45463	1	11335	5	NULL	NULL	NULL	NULL	TM2	GP		is mutated to			Ala-73		TM2	GP		Val		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_38_36513_s_192	12837756	A naturally occurring mutation in TM2, Ala-73 to Val has been shown to be associated with an increase in CCR5 binding affinity to RANTES and increased sensitivity to the induction of chemotaxis by this ligand ( ,  ).	bind
45465	2	11335	5	NULL	NULL	NULL	NULL	CCR5	GP		bind					RANTES	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_38_36513_s_192	12837756	A naturally occurring mutation in TM2, Ala-73 to Val has been shown to be associated with an increase in CCR5 binding affinity to RANTES and increased sensitivity to the induction of chemotaxis by this ligand ( ,  ).	bind
45466	3	11335	5	NULL	NULL	NULL	NULL	statement 1	Process		is associated with					statement 2	Process	increase in			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_38_36513_s_192	12837756	A naturally occurring mutation in TM2, Ala-73 to Val has been shown to be associated with an increase in CCR5 binding affinity to RANTES and increased sensitivity to the induction of chemotaxis by this ligand ( ,  ).	bind
45467	4	11335	5	NULL	NULL	NULL	NULL	RANTES	GP		induce					chemotaxis	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_38_36513_s_192	12837756	A naturally occurring mutation in TM2, Ala-73 to Val has been shown to be associated with an increase in CCR5 binding affinity to RANTES and increased sensitivity to the induction of chemotaxis by this ligand ( ,  ).	bind
45468	5	11335	5	NULL	NULL	NULL	NULL	statement 1	Process		is associated with					statement 4	Process	increased sensitivity to			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_38_36513_s_192	12837756	A naturally occurring mutation in TM2, Ala-73 to Val has been shown to be associated with an increase in CCR5 binding affinity to RANTES and increased sensitivity to the induction of chemotaxis by this ligand ( ,  ).	bind
45964	1	11335	6	NULL	NULL	0	NULL	CCR5	NULL		has affinity for	NULL				RANTES	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_38_36513_s_192	12837756	A naturally occurring mutation in TM2, Ala-73 to Val has been shown to be associated with an increase in CCR5 binding affinity to RANTES and increased sensitivity to the induction of chemotaxis by this ligand ( ,  ).	bind
45965	2	11335	6	NULL	NULL	0	NULL	TM2	NULL		is mutated to	NULL		Ala-73		TM2	NULL		Val		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_38_36513_s_192	12837756	A naturally occurring mutation in TM2, Ala-73 to Val has been shown to be associated with an increase in CCR5 binding affinity to RANTES and increased sensitivity to the induction of chemotaxis by this ligand ( ,  ).	bind
45966	3	11335	6	NULL	NULL	0	NULL	statement 2	NULL		is associated with	NULL				statement 1	NULL	increase in			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_38_36513_s_192	12837756	A naturally occurring mutation in TM2, Ala-73 to Val has been shown to be associated with an increase in CCR5 binding affinity to RANTES and increased sensitivity to the induction of chemotaxis by this ligand ( ,  ).	bind
51465	4	11335	6	10	NULL	0	NULL	RANTES	NULL		induce	NULL				chemotaxis	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_38_36513_s_192	12837756	A naturally occurring mutation in TM2, Ala-73 to Val has been shown to be associated with an increase in CCR5 binding affinity to RANTES and increased sensitivity to the induction of chemotaxis by this ligand ( ,  ).	bind
51466	5	11335	6	10	NULL	0	NULL	statement 2	NULL		is associated with	NULL				statement 4	NULL	increased sensitivity to			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_38_36513_s_192	12837756	A naturally occurring mutation in TM2, Ala-73 to Val has been shown to be associated with an increase in CCR5 binding affinity to RANTES and increased sensitivity to the induction of chemotaxis by this ligand ( ,  ).	bind
45469	1	11336	5	NULL	NULL	NULL	NULL	FGF	GP		is					fibroblast growth factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_gene_230_1_69_s_323	10196476	A naturally occurring secreted form of fibroblast growth factor (FGF) receptor 1 binds basic FGF in preference over acidic FGF.	bind
45470	2	11336	5	NULL	NULL	NULL	NULL	fibroblast growth factor receptor 1	GP	naturally occurring;;secreted	bind					FGF	GP	basic			NULL		NULL	NULL	NULL	NULL	gw60_gene_230_1_69_s_323	10196476	A naturally occurring secreted form of fibroblast growth factor (FGF) receptor 1 binds basic FGF in preference over acidic FGF.	bind
45471	3	11336	5	NULL	NULL	NULL	NULL	fibroblast growth factor receptor 1	GP	naturally occurring;;secreted	bind					FGF	GP	acidic			NULL		NULL	NULL	NULL	NULL	gw60_gene_230_1_69_s_323	10196476	A naturally occurring secreted form of fibroblast growth factor (FGF) receptor 1 binds basic FGF in preference over acidic FGF.	bind
45472	4	11336	5	NULL	NULL	NULL	NULL	statement 2	Process		is prefered over					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_gene_230_1_69_s_323	10196476	A naturally occurring secreted form of fibroblast growth factor (FGF) receptor 1 binds basic FGF in preference over acidic FGF.	bind
45967	1	11336	6	NULL	NULL	0	NULL	FGF	NULL		is	NULL				fibroblast growth factor	NULL				NULL		0	NULL	NULL	NULL	gw60_gene_230_1_69_s_323	10196476	A naturally occurring secreted form of fibroblast growth factor (FGF) receptor 1 binds basic FGF in preference over acidic FGF.	bind
45968	2	11336	6	10	NULL	0	NULL	FGF receptor 1	NULL	naturally occuring;; secreted form	bind	NULL				FGF	NULL	basic			NULL		NULL	NULL	NULL	NULL	gw60_gene_230_1_69_s_323	10196476	A naturally occurring secreted form of fibroblast growth factor (FGF) receptor 1 binds basic FGF in preference over acidic FGF.	bind
45969	3	11336	6	10	NULL	0	NULL	FGF receptor 1	NULL	naturally occuring;; secreted form	bind	NULL				FGF	NULL	acidic			NULL		NULL	NULL	NULL	NULL	gw60_gene_230_1_69_s_323	10196476	A naturally occurring secreted form of fibroblast growth factor (FGF) receptor 1 binds basic FGF in preference over acidic FGF.	bind
45970	4	11336	6	NULL	NULL	0	NULL	statement 2	NULL		is more preferential than	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_gene_230_1_69_s_323	10196476	A naturally occurring secreted form of fibroblast growth factor (FGF) receptor 1 binds basic FGF in preference over acidic FGF.	bind
45473	1	11337	5	NULL	NULL	NULL	NULL	Tcf3	GP		bind					beta-catenin	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_983_s_221	11524435	A nearly fivefold increase in the binding of Tcf3 to beta-catenin is seen when Tcf3 beads were preincubated with CK1epsilon.	bind
45474	2	11337	5	NULL	NULL	NULL	NULL	CK1epsilon	GP	presence of	increases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_983_s_221	11524435	A nearly fivefold increase in the binding of Tcf3 to beta-catenin is seen when Tcf3 beads were preincubated with CK1epsilon.	bind
45971	1	11337	6	NULL	NULL	0	NULL	Tcf3	NULL		bind	NULL				beta-catenin	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_154_5_983_s_221	11524435	A nearly fivefold increase in the binding of Tcf3 to beta-catenin is seen when Tcf3 beads were preincubated with CK1epsilon.	bind
45973	2	11337	6	10	NULL	0	NULL	CK1epsilon	NULL	presence of	increase	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_5_983_s_221	11524435	A nearly fivefold increase in the binding of Tcf3 to beta-catenin is seen when Tcf3 beads were preincubated with CK1epsilon.	bind
45475	1	11338	5	NULL	NULL	NULL	NULL				bind				GC-box motif	Sp1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4293_s_232	12024040	A nearly perfect GC-box motif bound Sp1 and Sp3, as judged by electrophoretic mobility shift assays and supershifts with the appropriate antibodies (Fig.  7A).	bind
45476	2	11338	5	NULL	NULL	NULL	NULL				bind				GC-box motif	Sp3	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_12_4293_s_232	12024040	A nearly perfect GC-box motif bound Sp1 and Sp3, as judged by electrophoretic mobility shift assays and supershifts with the appropriate antibodies (Fig.  7A).	bind
45974	1	11338	6	NULL	NULL	0	NULL	Sp1	NULL		bind	NULL					NULL			GC-box 	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_12_4293_s_232	12024040	A nearly perfect GC-box motif bound Sp1 and Sp3, as judged by electrophoretic mobility shift assays and supershifts with the appropriate antibodies (Fig.  7A).	bind
45975	2	11338	6	NULL	NULL	0	NULL	Sp3	NULL		bind	NULL					NULL			GC-box	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_12_4293_s_232	12024040	A nearly perfect GC-box motif bound Sp1 and Sp3, as judged by electrophoretic mobility shift assays and supershifts with the appropriate antibodies (Fig.  7A).	bind
45477	1	11339	5	NULL	NULL	NULL	NULL	toxin A	GP		bind					enterocyte receptors	GP	luminal			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_98_3_641_s_23	8698855	A necessary  first step for enterotoxicity is binding of toxin A to luminal enterocyte receptors.	bind
45478	2	11339	5	NULL	NULL	NULL	NULL	statement 1	Process		is first step for		necessary			enterotoxicity	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_98_3_641_s_23	8698855	A necessary  first step for enterotoxicity is binding of toxin A to luminal enterocyte receptors.	bind
45976	1	11339	6	NULL	NULL	0	NULL	toxin A	NULL		bind	NULL				enterocyte receptor	NULL	luminal			NULL		0	NULL	NULL	NULL	gw60_jclininvest_98_3_641_s_23	8698855	A necessary  first step for enterotoxicity is binding of toxin A to luminal enterocyte receptors.	bind
45479	1	11340	5	NULL	NULL	NULL	NULL	CETP	GP		bind		stably			HDL	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_718_s_215	10073979	A necessary corollary to these findings is that the often-reported stable binding of CETP to HDL does not result in selective transfer from this lipoprotein fraction.	bind
45480	2	11340	5	NULL	NULL	NULL	NULL	statement 1	Process		does not result in					lipoprotein	GP	selective transfer from;;fraction of			NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_718_s_215	10073979	A necessary corollary to these findings is that the often-reported stable binding of CETP to HDL does not result in selective transfer from this lipoprotein fraction.	bind
51467	3	11340	5	NULL	NULL	NULL	NULL	HDL	GP		is a type of					lipoprotein	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_718_s_215	10073979	A necessary corollary to these findings is that the often-reported stable binding of CETP to HDL does not result in selective transfer from this lipoprotein fraction.	bind
45977	1	11340	6	10	NULL	0	NULL	CETP			bind		stable			HDL					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_718_s_215	10073979	A necessary corollary to these findings is that the often-reported stable binding of CETP to HDL does not result in selective transfer from this lipoprotein fraction.	bind
45978	2	11340	6	NULL	NULL	0	NULL	statement 1	NULL		does not result in	NULL				HDL	NULL	transfer from			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_718_s_215	10073979	A necessary corollary to these findings is that the often-reported stable binding of CETP to HDL does not result in selective transfer from this lipoprotein fraction.	bind
45979	3	11340	6	10	NULL	0	NULL	HDL	NULL		is a type of	NULL				lipoprotein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_3_718_s_215	10073979	A necessary corollary to these findings is that the often-reported stable binding of CETP to HDL does not result in selective transfer from this lipoprotein fraction.	bind
45481	1	11341	5	NULL	NULL	NULL	NULL	TRA-2	GP		bind		directly			FEM-3	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_34_12549_s_201	15306688	A negative arrow from TRA-2 to FEM-3 reflects the possibility  that TRA-2 directly binds and inhibits FEM-3 ( ).	bind
45482	2	11341	5	NULL	NULL	NULL	NULL	statement 1	Process		inhibit					FEM-3	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_34_12549_s_201	15306688	A negative arrow from TRA-2 to FEM-3 reflects the possibility  that TRA-2 directly binds and inhibits FEM-3 ( ).	bind
45980	1	11341	6	NULL	NULL	0	NULL	TRA-2	NULL		bind	NULL	directly			FEM-3	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_101_34_12549_s_201	15306688	A negative arrow from TRA-2 to FEM-3 reflects the possibility  that TRA-2 directly binds and inhibits FEM-3 ( ).	bind
45981	2	11341	6	NULL	NULL	0	NULL	TRA-2	NULL		inhibits	NULL				FEM-3	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_101_34_12549_s_201	15306688	A negative arrow from TRA-2 to FEM-3 reflects the possibility  that TRA-2 directly binds and inhibits FEM-3 ( ).	bind
45483	1	11342	5	NULL	NULL	NULL	NULL	CHO cells	Cell		is transfected with					P-selectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_14_1710_s_87	11015352	A negative control experiment using an isotype-matched control revealed that the binding of HL-60 cells to P-selectin - transfected CHO cells was hardly suppressed compared with results for S789G (Table  ).	bind
45484	2	11342	5	NULL	NULL	NULL	NULL	HL-60 cells	Cell		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulation_102_14_1710_s_87	11015352	A negative control experiment using an isotype-matched control revealed that the binding of HL-60 cells to P-selectin - transfected CHO cells was hardly suppressed compared with results for S789G (Table  ).	bind
45982	1	11342	6	NULL	NULL	0	NULL	P-selectin	NULL		is transfected to	NULL				CHO cells	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_102_14_1710_s_87	11015352	A negative control experiment using an isotype-matched control revealed that the binding of HL-60 cells to P-selectin - transfected CHO cells was hardly suppressed compared with results for S789G (Table  ).	bind
45983	2	11342	6	NULL	NULL	0	NULL	HL-60 cells	NULL		bind	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_circulation_102_14_1710_s_87	11015352	A negative control experiment using an isotype-matched control revealed that the binding of HL-60 cells to P-selectin - transfected CHO cells was hardly suppressed compared with results for S789G (Table  ).	bind
45485	1	11343	5	NULL	NULL	NULL	NULL	Grb-2	GP		bind		low affinity			CD3-epsilon-ITAM	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_40_25310_s_176	9312149	A negative control in these experiments was the comparison with the low affinity binding of Grb-2 to CD3-epsilon-ITAM ( 37).	bind
45984	1	11343	6	NULL	NULL	0	NULL	Grb-2	NULL		bind	NULL	low affinity			CD3-epsilon-ITAM	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_40_25310_s_176	9312149	A negative control in these experiments was the comparison with the low affinity binding of Grb-2 to CD3-epsilon-ITAM ( 37).	bind
45487	1	11345	5	NULL	NULL	NULL	NULL	parathyroid hormone-related peptide gene	GP	human	bind				negative Vitamin D response DNA element	Vitamin D receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_27_16310_s_256	8663213	A Negative Vitamin D Response DNA Element in the Human Parathyroid Hormone-related Peptide Gene Binds to Vitamin D Receptor Along with Ku Antigen to Mediate Negative Gene Regulation by Vitamin D.   J. Biol.	bind
45488	2	11345	5	NULL	NULL	NULL	NULL	parathyroid hormone-related peptide gene	GP	human	bind				negative Vitamin D response DNA element	Ku Antigen	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_27_16310_s_256	8663213	A Negative Vitamin D Response DNA Element in the Human Parathyroid Hormone-related Peptide Gene Binds to Vitamin D Receptor Along with Ku Antigen to Mediate Negative Gene Regulation by Vitamin D.   J. Biol.	bind
45489	3	11345	5	NULL	NULL	NULL	NULL	Vitamin D	Chemical		mediate					negative gene regulation	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_27_16310_s_256	8663213	A Negative Vitamin D Response DNA Element in the Human Parathyroid Hormone-related Peptide Gene Binds to Vitamin D Receptor Along with Ku Antigen to Mediate Negative Gene Regulation by Vitamin D.   J. Biol.	bind
45490	4	11345	5	NULL	NULL	NULL	NULL	statement 1	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_27_16310_s_256	8663213	A Negative Vitamin D Response DNA Element in the Human Parathyroid Hormone-related Peptide Gene Binds to Vitamin D Receptor Along with Ku Antigen to Mediate Negative Gene Regulation by Vitamin D.   J. Biol.	bind
45491	5	11345	5	NULL	NULL	NULL	NULL	statement 2	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_27_16310_s_256	8663213	A Negative Vitamin D Response DNA Element in the Human Parathyroid Hormone-related Peptide Gene Binds to Vitamin D Receptor Along with Ku Antigen to Mediate Negative Gene Regulation by Vitamin D.   J. Biol.	bind
45985	1	11345	6	NULL	NULL	0	NULL	Parathyroid Hormone-related Peptide Gene	NULL	human	bind	NULL			Vitamin D Response DNA Element	Vitamin D Receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_27_16310_s_256	8663213	A Negative Vitamin D Response DNA Element in the Human Parathyroid Hormone-related Peptide Gene Binds to Vitamin D Receptor Along with Ku Antigen to Mediate Negative Gene Regulation by Vitamin D.   J. Biol.	bind
45986	2	11345	6	10	NULL	0	NULL	Parathyroid Hormone-related Peptide Gene	NULL	human	bind	NULL			Vitamin D Response DNA Element	Ku antigen	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_27_16310_s_256	8663213	A Negative Vitamin D Response DNA Element in the Human Parathyroid Hormone-related Peptide Gene Binds to Vitamin D Receptor Along with Ku Antigen to Mediate Negative Gene Regulation by Vitamin D.   J. Biol.	bind
45987	5	11345	6	10	NULL	0	NULL	statement 2	NULL		mediates	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_27_16310_s_256	8663213	A Negative Vitamin D Response DNA Element in the Human Parathyroid Hormone-related Peptide Gene Binds to Vitamin D Receptor Along with Ku Antigen to Mediate Negative Gene Regulation by Vitamin D.   J. Biol.	bind
45988	3	11345	6	10	NULL	0	NULL	vitamin D 	NULL		causes	NULL				gene regulation	NULL	negative			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_27_16310_s_256	8663213	A Negative Vitamin D Response DNA Element in the Human Parathyroid Hormone-related Peptide Gene Binds to Vitamin D Receptor Along with Ku Antigen to Mediate Negative Gene Regulation by Vitamin D.   J. Biol.	bind
45989	4	11345	6	10	NULL	0	NULL	statement 1	NULL		mediates	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_27_16310_s_256	8663213	A Negative Vitamin D Response DNA Element in the Human Parathyroid Hormone-related Peptide Gene Binds to Vitamin D Receptor Along with Ku Antigen to Mediate Negative Gene Regulation by Vitamin D.   J. Biol.	bind
45492	1	11349	5	NULL	NULL	NULL	NULL	Pd(II) nanoparticle catalyst	Chemical	negatively charged	bind					PEI layer	Chemical	terminal cationic 			NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_j-am-chem-soc_125_37_16220946_s_4	16220946	A negatively charged Pd(II) nanoparticle catalyst  is bound to the terminal cationic PEI layer of the multilayer film and  initiates selective template metallization to form the helical Cu nanostructures.	bind
45493	2	11349	5	NULL	NULL	NULL	NULL	statement 1	Process		initiates					template metallization	Process	selective			NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_j-am-chem-soc_125_37_16220946_s_4	16220946	A negatively charged Pd(II) nanoparticle catalyst  is bound to the terminal cationic PEI layer of the multilayer film and  initiates selective template metallization to form the helical Cu nanostructures.	bind
45494	3	11349	5	NULL	NULL	NULL	NULL	statement 2	Process		forms					helical Cu nanostructures	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_j-am-chem-soc_125_37_16220946_s_4	16220946	A negatively charged Pd(II) nanoparticle catalyst  is bound to the terminal cationic PEI layer of the multilayer film and  initiates selective template metallization to form the helical Cu nanostructures.	bind
46107	1	11349	6	NULL	NULL	0	NULL	Pd(II) nanoparticle catalyst	NULL	negatively charged	bind	NULL				PEI layer	NULL	terminal cationic			NULL		0	NULL	NULL	NULL	abs-batch0530-0539_j-am-chem-soc_125_37_16220946_s_4	16220946	A negatively charged Pd(II) nanoparticle catalyst  is bound to the terminal cationic PEI layer of the multilayer film and  initiates selective template metallization to form the helical Cu nanostructures.	bind
46108	2	11349	6	NULL	NULL	0	NULL	statement 1	NULL		initiates	NULL				template metallization	NULL				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_j-am-chem-soc_125_37_16220946_s_4	16220946	A negatively charged Pd(II) nanoparticle catalyst  is bound to the terminal cationic PEI layer of the multilayer film and  initiates selective template metallization to form the helical Cu nanostructures.	bind
46115	3	11349	6	10	NULL	0	NULL	statement 2	NULL		forms	NULL				helical Cu nanostructures	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_j-am-chem-soc_125_37_16220946_s_4	16220946	A negatively charged Pd(II) nanoparticle catalyst  is bound to the terminal cationic PEI layer of the multilayer film and  initiates selective template metallization to form the helical Cu nanostructures.	bind
45495	1	11350	5	NULL	NULL	NULL	NULL	PS	Chemical	negatively charged	bind		specifically			annexin V	GP	fluorescently labeled			NULL		NULL	NULL	NULL	NULL	gw60_febslett_477_1_1_s_22	10899301	A negatively charged PS can specifically bind fluorescently labeled annexin V, the most commonly used reagent for flow cytometric measurements of apoptosis [  11 and   12].	bind
45990	1	11350	6	NULL	NULL	0	NULL	PS	NULL	negatively charged	bind	NULL	specifically			annexin V	NULL	fluorescently labeled			NULL		0	NULL	NULL	NULL	gw60_febslett_477_1_1_s_22	10899301	A negatively charged PS can specifically bind fluorescently labeled annexin V, the most commonly used reagent for flow cytometric measurements of apoptosis [  11 and   12].	bind
45502	1	11352	5	NULL	NULL	NULL	NULL	hnRNP H	GP		bind									enhancer	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_35_32943_s_21	12826680	A neurally enriched homologue of PTB  also greatly enhances the binding of hnRNP H and KH-type splicing-regulatory  protein to the enhancer ( ).	bind
45503	2	11352	5	NULL	NULL	NULL	NULL	KH-type splicing-regulatory protein	GP		bind									enhancer	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_35_32943_s_21	12826680	A neurally enriched homologue of PTB  also greatly enhances the binding of hnRNP H and KH-type splicing-regulatory  protein to the enhancer ( ).	bind
45504	3	11352	5	NULL	NULL	NULL	NULL	PTB homolog	GP	neurally enriched	enhance		greatly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_35_32943_s_21	12826680	A neurally enriched homologue of PTB  also greatly enhances the binding of hnRNP H and KH-type splicing-regulatory  protein to the enhancer ( ).	bind
45505	4	11352	5	NULL	NULL	NULL	NULL	PTB homolog	GP	neurally enriched	enhance		greatly			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_35_32943_s_21	12826680	A neurally enriched homologue of PTB  also greatly enhances the binding of hnRNP H and KH-type splicing-regulatory  protein to the enhancer ( ).	bind
45991	1	11352	6	NULL	NULL	0	NULL	hnRNP H	NULL		bind	NULL					NULL			enhancer	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_35_32943_s_21	12826680	A neurally enriched homologue of PTB  also greatly enhances the binding of hnRNP H and KH-type splicing-regulatory  protein to the enhancer ( ).	bind
45992	2	11352	6	NULL	NULL	0	NULL	KH-type splicing-regulatory protein	NULL		bind	NULL					NULL			enhancer	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_35_32943_s_21	12826680	A neurally enriched homologue of PTB  also greatly enhances the binding of hnRNP H and KH-type splicing-regulatory  protein to the enhancer ( ).	bind
45993	3	11352	6	10	NULL	0	NULL	PTB homologue		neurally enriched	enhances		greatly			statement 1					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_35_32943_s_21	12826680	A neurally enriched homologue of PTB  also greatly enhances the binding of hnRNP H and KH-type splicing-regulatory  protein to the enhancer ( ).	bind
45994	4	11352	6	10	NULL	0	NULL	PTB homologue		neurally enriched	enhances		greatly			statement 2					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_35_32943_s_21	12826680	A neurally enriched homologue of PTB  also greatly enhances the binding of hnRNP H and KH-type splicing-regulatory  protein to the enhancer ( ).	bind
45506	1	11353	5	NULL	NULL	NULL	NULL	neurobeachin isoform	GP		does not bind					RII	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_20_23_8551_s_8	11102458	A neurobeachin isoform that does not bind RII, beige-like protein (BGL), is expressed in many tissues.	bind
45507	2	11353	5	NULL	NULL	NULL	NULL	neurobeachin isoform	GP		does not bind					BGL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_20_23_8551_s_8	11102458	A neurobeachin isoform that does not bind RII, beige-like protein (BGL), is expressed in many tissues.	bind
45508	3	11353	5	NULL	NULL	NULL	NULL	BGL	GP		is					beige-like protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_20_23_8551_s_8	11102458	A neurobeachin isoform that does not bind RII, beige-like protein (BGL), is expressed in many tissues.	bind
45995	1	11353	6	NULL	NULL	0	NULL	neurobeachin isoform	NULL		does not bind	NULL				RII	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_23_8551_s_8	11102458	A neurobeachin isoform that does not bind RII, beige-like protein (BGL), is expressed in many tissues.	bind
45996	2	11353	6	10	NULL	0	NULL	neurobeachin isoform	NULL		does not bind	NULL				BGL	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_20_23_8551_s_8	11102458	A neurobeachin isoform that does not bind RII, beige-like protein (BGL), is expressed in many tissues.	bind
45997	3	11353	6	NULL	NULL	0	NULL	BGL	NULL		is	NULL				beige-like protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_23_8551_s_8	11102458	A neurobeachin isoform that does not bind RII, beige-like protein (BGL), is expressed in many tissues.	bind
45511	1	11354	5	NULL	NULL	NULL	NULL	neuroligin	GP		is a type of					neuronal cell adhesion molecule	GP				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_22_3_757_s_22	11826105	A neuronal cell adhesion molecule, neuroligin, and a GDP/GTP exchange factor for rap1 bind to the second PDZ domain (PDZ1) (Hirao et al., 1998  ; Ohtsuka et al., 1999  ).	bind
45512	2	11354	5	NULL	NULL	NULL	NULL	neuroligin	GP		bind								PDZ1		NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_22_3_757_s_22	11826105	A neuronal cell adhesion molecule, neuroligin, and a GDP/GTP exchange factor for rap1 bind to the second PDZ domain (PDZ1) (Hirao et al., 1998  ; Ohtsuka et al., 1999  ).	bind
45513	3	11354	5	NULL	NULL	NULL	NULL	PDZ1	AminoAcid		is					second PDZ domain	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_22_3_757_s_22	11826105	A neuronal cell adhesion molecule, neuroligin, and a GDP/GTP exchange factor for rap1 bind to the second PDZ domain (PDZ1) (Hirao et al., 1998  ; Ohtsuka et al., 1999  ).	bind
45514	4	11354	5	NULL	NULL	NULL	NULL	GDP/GTP exchange factor for rap1	GP		bind								PDZ1		NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_22_3_757_s_22	11826105	A neuronal cell adhesion molecule, neuroligin, and a GDP/GTP exchange factor for rap1 bind to the second PDZ domain (PDZ1) (Hirao et al., 1998  ; Ohtsuka et al., 1999  ).	bind
45998	1	11354	6	NULL	NULL	0	NULL	neuroligin	NULL		is a type of	NULL				neuronal cell adhesion molecule	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_22_3_757_s_22	11826105	A neuronal cell adhesion molecule, neuroligin, and a GDP/GTP exchange factor for rap1 bind to the second PDZ domain (PDZ1) (Hirao et al., 1998  ; Ohtsuka et al., 1999  ).	bind
45999	2	11354	6	NULL	NULL	0	NULL	neuroligin	NULL		bind	NULL					NULL		PDZ1		NULL		0	NULL	NULL	NULL	gw60_jneurosci_22_3_757_s_22	11826105	A neuronal cell adhesion molecule, neuroligin, and a GDP/GTP exchange factor for rap1 bind to the second PDZ domain (PDZ1) (Hirao et al., 1998  ; Ohtsuka et al., 1999  ).	bind
46000	3	11354	6	NULL	NULL	0	NULL	GDP/GTP exchange factor for rap1	NULL		bind	NULL					NULL		PDZ1		NULL		0	NULL	NULL	NULL	gw60_jneurosci_22_3_757_s_22	11826105	A neuronal cell adhesion molecule, neuroligin, and a GDP/GTP exchange factor for rap1 bind to the second PDZ domain (PDZ1) (Hirao et al., 1998  ; Ohtsuka et al., 1999  ).	bind
46001	4	11354	6	NULL	NULL	0	NULL	PDZ1	NULL		is	NULL				second PDZ domain 	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_22_3_757_s_22	11826105	A neuronal cell adhesion molecule, neuroligin, and a GDP/GTP exchange factor for rap1 bind to the second PDZ domain (PDZ1) (Hirao et al., 1998  ; Ohtsuka et al., 1999  ).	bind
45515	1	11355	5	NULL	NULL	NULL	NULL	Hsp70	GP		bind					DC	Cell				NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_3_353_s_64	12354387	A neutralizing anti-CD14 mAb (clone MY4) did not modulate Hsp70 binding to DC or macrophages   (Table 1), and Hsp70 did not bind to CD14-transfected cells   (Figure 2) .	bind
45516	2	11355	5	NULL	NULL	NULL	NULL	Hsp70	GP		bind					macrophages	Cell				NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_3_353_s_64	12354387	A neutralizing anti-CD14 mAb (clone MY4) did not modulate Hsp70 binding to DC or macrophages   (Table 1), and Hsp70 did not bind to CD14-transfected cells   (Figure 2) .	bind
45517	3	11355	5	NULL	NULL	NULL	NULL	anti-CD14 mAb	GP	neutralizing	does not modulate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_3_353_s_64	12354387	A neutralizing anti-CD14 mAb (clone MY4) did not modulate Hsp70 binding to DC or macrophages   (Table 1), and Hsp70 did not bind to CD14-transfected cells   (Figure 2) .	bind
45518	4	11355	5	NULL	NULL	NULL	NULL	anti-CD14 mAb	GP	neutralizing	does not modulate					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_3_353_s_64	12354387	A neutralizing anti-CD14 mAb (clone MY4) did not modulate Hsp70 binding to DC or macrophages   (Table 1), and Hsp70 did not bind to CD14-transfected cells   (Figure 2) .	bind
45519	5	11355	5	NULL	NULL	NULL	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_3_353_s_64	12354387	A neutralizing anti-CD14 mAb (clone MY4) did not modulate Hsp70 binding to DC or macrophages   (Table 1), and Hsp70 did not bind to CD14-transfected cells   (Figure 2) .	bind
45520	7	11355	5	NULL	NULL	NULL	NULL	Hsp70	GP		does not bind					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_3_353_s_64	12354387	A neutralizing anti-CD14 mAb (clone MY4) did not modulate Hsp70 binding to DC or macrophages   (Table 1), and Hsp70 did not bind to CD14-transfected cells   (Figure 2) .	bind
45521	6	11355	5	NULL	NULL	NULL	NULL	cells	Cell		is transfected with					CD14	GP				NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_3_353_s_64	12354387	A neutralizing anti-CD14 mAb (clone MY4) did not modulate Hsp70 binding to DC or macrophages   (Table 1), and Hsp70 did not bind to CD14-transfected cells   (Figure 2) .	bind
46002	1	11355	6	NULL	NULL	0	NULL	Hsp70	NULL		bind	NULL				DC	NULL				NULL		0	NULL	NULL	NULL	gw60_immunity_17_3_353_s_64	12354387	A neutralizing anti-CD14 mAb (clone MY4) did not modulate Hsp70 binding to DC or macrophages   (Table 1), and Hsp70 did not bind to CD14-transfected cells   (Figure 2) .	bind
46003	2	11355	6	NULL	NULL	0	NULL	Hsp70	NULL		bind	NULL				macrophages	NULL				NULL		0	NULL	NULL	NULL	gw60_immunity_17_3_353_s_64	12354387	A neutralizing anti-CD14 mAb (clone MY4) did not modulate Hsp70 binding to DC or macrophages   (Table 1), and Hsp70 did not bind to CD14-transfected cells   (Figure 2) .	bind
46004	3	11355	6	NULL	NULL	0	NULL	anti-CD14 mAb	NULL	neutralizing	did not modulate	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_immunity_17_3_353_s_64	12354387	A neutralizing anti-CD14 mAb (clone MY4) did not modulate Hsp70 binding to DC or macrophages   (Table 1), and Hsp70 did not bind to CD14-transfected cells   (Figure 2) .	bind
46005	4	11355	6	NULL	NULL	0	NULL	anti-CD14 mAb	NULL	neutralizing	did not modulate	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_immunity_17_3_353_s_64	12354387	A neutralizing anti-CD14 mAb (clone MY4) did not modulate Hsp70 binding to DC or macrophages   (Table 1), and Hsp70 did not bind to CD14-transfected cells   (Figure 2) .	bind
46006	6	11355	6	10	NULL	0	NULL	Hsp70	NULL		does not bind	NULL				statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw60_immunity_17_3_353_s_64	12354387	A neutralizing anti-CD14 mAb (clone MY4) did not modulate Hsp70 binding to DC or macrophages   (Table 1), and Hsp70 did not bind to CD14-transfected cells   (Figure 2) .	bind
51489	5	11355	6	10	NULL	0	NULL	cells	NULL		transfected with	NULL				CD14	NULL				NULL		0	NULL	NULL	NULL	gw60_immunity_17_3_353_s_64	12354387	A neutralizing anti-CD14 mAb (clone MY4) did not modulate Hsp70 binding to DC or macrophages   (Table 1), and Hsp70 did not bind to CD14-transfected cells   (Figure 2) .	bind
51490	7	11355	6	10	NULL	0	NULL	statement 3	NULL		is an alternative to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_immunity_17_3_353_s_64	12354387	A neutralizing anti-CD14 mAb (clone MY4) did not modulate Hsp70 binding to DC or macrophages   (Table 1), and Hsp70 did not bind to CD14-transfected cells   (Figure 2) .	bind
45522	1	11356	5	NULL	NULL	NULL	NULL	LDL	GP	Oxidized	bind					LOX-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_511_1_133_s_97	11821063	A neutralizing anti-LOX-1 monoclonal antibody, which inhibits binding of oxidized LDL to LOX-1, partly (by 72% of the LOX-1-dependent adhesion) but significantly inhibited adhesion of THP-1 cells to CHO-K1 cells stably expressing bovine LOX-1 (bLOX-1-CHO).	bind
45523	2	11356	5	NULL	NULL	NULL	NULL	anti-LOX-1	GP		is a type of					monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_511_1_133_s_97	11821063	A neutralizing anti-LOX-1 monoclonal antibody, which inhibits binding of oxidized LDL to LOX-1, partly (by 72% of the LOX-1-dependent adhesion) but significantly inhibited adhesion of THP-1 cells to CHO-K1 cells stably expressing bovine LOX-1 (bLOX-1-CHO).	bind
45524	3	11356	5	NULL	NULL	NULL	NULL	anti-LOX-1	GP	neutralizing	inhibit		partly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_511_1_133_s_97	11821063	A neutralizing anti-LOX-1 monoclonal antibody, which inhibits binding of oxidized LDL to LOX-1, partly (by 72% of the LOX-1-dependent adhesion) but significantly inhibited adhesion of THP-1 cells to CHO-K1 cells stably expressing bovine LOX-1 (bLOX-1-CHO).	bind
45525	4	11356	5	NULL	NULL	NULL	NULL	CHO-K1 cells	Cell		express		stably			LOX-1	GP	bovine			NULL		NULL	NULL	NULL	NULL	gw60_febslett_511_1_133_s_97	11821063	A neutralizing anti-LOX-1 monoclonal antibody, which inhibits binding of oxidized LDL to LOX-1, partly (by 72% of the LOX-1-dependent adhesion) but significantly inhibited adhesion of THP-1 cells to CHO-K1 cells stably expressing bovine LOX-1 (bLOX-1-CHO).	bind
45526	5	11356	5	NULL	NULL	NULL	NULL	bLOX-1-CHO	Cell		is					statement 4	Cell				NULL		NULL	NULL	NULL	NULL	gw60_febslett_511_1_133_s_97	11821063	A neutralizing anti-LOX-1 monoclonal antibody, which inhibits binding of oxidized LDL to LOX-1, partly (by 72% of the LOX-1-dependent adhesion) but significantly inhibited adhesion of THP-1 cells to CHO-K1 cells stably expressing bovine LOX-1 (bLOX-1-CHO).	bind
45527	6	11356	5	NULL	NULL	NULL	NULL	THP-1 cells	Cell		adhere to					bLOX-1-CHO	Cell				NULL		NULL	NULL	NULL	NULL	gw60_febslett_511_1_133_s_97	11821063	A neutralizing anti-LOX-1 monoclonal antibody, which inhibits binding of oxidized LDL to LOX-1, partly (by 72% of the LOX-1-dependent adhesion) but significantly inhibited adhesion of THP-1 cells to CHO-K1 cells stably expressing bovine LOX-1 (bLOX-1-CHO).	bind
45528	7	11356	5	NULL	NULL	NULL	NULL	anti-LOX-1	GP	neutralizing	inhibit		significantly			statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_511_1_133_s_97	11821063	A neutralizing anti-LOX-1 monoclonal antibody, which inhibits binding of oxidized LDL to LOX-1, partly (by 72% of the LOX-1-dependent adhesion) but significantly inhibited adhesion of THP-1 cells to CHO-K1 cells stably expressing bovine LOX-1 (bLOX-1-CHO).	bind
46007	1	11356	6	NULL	NULL	0	NULL	LDL	NULL	oxidized	bind	NULL				LOX-1	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_511_1_133_s_97	11821063	A neutralizing anti-LOX-1 monoclonal antibody, which inhibits binding of oxidized LDL to LOX-1, partly (by 72% of the LOX-1-dependent adhesion) but significantly inhibited adhesion of THP-1 cells to CHO-K1 cells stably expressing bovine LOX-1 (bLOX-1-CHO).	bind
46008	2	11356	6	10	NULL	0	NULL	anti-LOX-1	NULL	neutralizing	inhibits	NULL	partly			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_febslett_511_1_133_s_97	11821063	A neutralizing anti-LOX-1 monoclonal antibody, which inhibits binding of oxidized LDL to LOX-1, partly (by 72% of the LOX-1-dependent adhesion) but significantly inhibited adhesion of THP-1 cells to CHO-K1 cells stably expressing bovine LOX-1 (bLOX-1-CHO).	bind
46009	3	11356	6	NULL	NULL	0	NULL	THP-1 cells	NULL		adhers to	NULL				bLOX-1-CHO	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_511_1_133_s_97	11821063	A neutralizing anti-LOX-1 monoclonal antibody, which inhibits binding of oxidized LDL to LOX-1, partly (by 72% of the LOX-1-dependent adhesion) but significantly inhibited adhesion of THP-1 cells to CHO-K1 cells stably expressing bovine LOX-1 (bLOX-1-CHO).	bind
46010	4	11356	6	NULL	NULL	0	NULL	CHO-K1 cells	NULL		express 	NULL	stably			LOX-1	NULL	bovine			NULL		0	NULL	NULL	NULL	gw60_febslett_511_1_133_s_97	11821063	A neutralizing anti-LOX-1 monoclonal antibody, which inhibits binding of oxidized LDL to LOX-1, partly (by 72% of the LOX-1-dependent adhesion) but significantly inhibited adhesion of THP-1 cells to CHO-K1 cells stably expressing bovine LOX-1 (bLOX-1-CHO).	bind
46011	5	11356	6	NULL	NULL	0	NULL	bLOX-1-CHO	NULL		is	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_511_1_133_s_97	11821063	A neutralizing anti-LOX-1 monoclonal antibody, which inhibits binding of oxidized LDL to LOX-1, partly (by 72% of the LOX-1-dependent adhesion) but significantly inhibited adhesion of THP-1 cells to CHO-K1 cells stably expressing bovine LOX-1 (bLOX-1-CHO).	bind
51500	6	11356	6	10	NULL	0	NULL	 anti-LOX-1 	NULL	neutralizing 	inhibit	NULL	significantly			statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_febslett_511_1_133_s_97	11821063	A neutralizing anti-LOX-1 monoclonal antibody, which inhibits binding of oxidized LDL to LOX-1, partly (by 72% of the LOX-1-dependent adhesion) but significantly inhibited adhesion of THP-1 cells to CHO-K1 cells stably expressing bovine LOX-1 (bLOX-1-CHO).	bind
51501	7	11356	6	10	NULL	0	NULL	anti-LOX-1	NULL		is a type of	NULL				monoclonal antibody	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_511_1_133_s_97	11821063	A neutralizing anti-LOX-1 monoclonal antibody, which inhibits binding of oxidized LDL to LOX-1, partly (by 72% of the LOX-1-dependent adhesion) but significantly inhibited adhesion of THP-1 cells to CHO-K1 cells stably expressing bovine LOX-1 (bLOX-1-CHO).	bind
45529	1	11357	5	NULL	NULL	NULL	NULL	 antibody	GP	neutralizing	reacts with					gp42	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-virol_72_1_9420211_s_4	9420211	A neutralizing antibody  that reacts with gp42 inhibits virus-cell fusion and blocks binding of  gp42 to HLA class II; antibody to HLA class II can inhibit infection,  and B cells that lack HLA class II can only be infected if HLA class II  expression is restored.	bind
45530	2	11357	5	NULL	NULL	NULL	NULL	statement 1	Process		inhibit					virus-cell fusion	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-virol_72_1_9420211_s_4	9420211	A neutralizing antibody  that reacts with gp42 inhibits virus-cell fusion and blocks binding of  gp42 to HLA class II; antibody to HLA class II can inhibit infection,  and B cells that lack HLA class II can only be infected if HLA class II  expression is restored.	bind
45531	3	11357	5	NULL	NULL	NULL	NULL	gp42	GP		bind					HLA class II	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-virol_72_1_9420211_s_4	9420211	A neutralizing antibody  that reacts with gp42 inhibits virus-cell fusion and blocks binding of  gp42 to HLA class II; antibody to HLA class II can inhibit infection,  and B cells that lack HLA class II can only be infected if HLA class II  expression is restored.	bind
45532	4	11357	5	NULL	NULL	NULL	NULL	statement 1	Process		block					statement 3	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-virol_72_1_9420211_s_4	9420211	A neutralizing antibody  that reacts with gp42 inhibits virus-cell fusion and blocks binding of  gp42 to HLA class II; antibody to HLA class II can inhibit infection,  and B cells that lack HLA class II can only be infected if HLA class II  expression is restored.	bind
45533	5	11357	5	NULL	NULL	NULL	NULL	antibody to HLA class II	GP		inhibit					infection	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-virol_72_1_9420211_s_4	9420211	A neutralizing antibody  that reacts with gp42 inhibits virus-cell fusion and blocks binding of  gp42 to HLA class II; antibody to HLA class II can inhibit infection,  and B cells that lack HLA class II can only be infected if HLA class II  expression is restored.	bind
45534	6	11357	5	NULL	NULL	NULL	NULL	B cells	Cell		lacks					HLA class II	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-virol_72_1_9420211_s_4	9420211	A neutralizing antibody  that reacts with gp42 inhibits virus-cell fusion and blocks binding of  gp42 to HLA class II; antibody to HLA class II can inhibit infection,  and B cells that lack HLA class II can only be infected if HLA class II  expression is restored.	bind
45535	7	11357	5	NULL	NULL	NULL	NULL	statement 6	Process	infection of	occurs on		only			HLA class II	GP	restoration of;;expression of			NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-virol_72_1_9420211_s_4	9420211	A neutralizing antibody  that reacts with gp42 inhibits virus-cell fusion and blocks binding of  gp42 to HLA class II; antibody to HLA class II can inhibit infection,  and B cells that lack HLA class II can only be infected if HLA class II  expression is restored.	bind
46012	1	11357	6	NULL	NULL	0	NULL	gp42	NULL		bind	NULL				HLA class II	NULL				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_j-virol_72_1_9420211_s_4	9420211	A neutralizing antibody  that reacts with gp42 inhibits virus-cell fusion and blocks binding of  gp42 to HLA class II; antibody to HLA class II can inhibit infection,  and B cells that lack HLA class II can only be infected if HLA class II  expression is restored.	bind
46013	2	11357	6	NULL	NULL	0	NULL	neutralizing antibody	NULL		reacts with	NULL				gp42	NULL				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_j-virol_72_1_9420211_s_4	9420211	A neutralizing antibody  that reacts with gp42 inhibits virus-cell fusion and blocks binding of  gp42 to HLA class II; antibody to HLA class II can inhibit infection,  and B cells that lack HLA class II can only be infected if HLA class II  expression is restored.	bind
46014	3	11357	6	NULL	NULL	0	NULL	statement 2	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_j-virol_72_1_9420211_s_4	9420211	A neutralizing antibody  that reacts with gp42 inhibits virus-cell fusion and blocks binding of  gp42 to HLA class II; antibody to HLA class II can inhibit infection,  and B cells that lack HLA class II can only be infected if HLA class II  expression is restored.	bind
46015	4	11357	6	NULL	NULL	0	NULL	statement 2	NULL		inhibits	NULL				virus-cell fusion	NULL				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_j-virol_72_1_9420211_s_4	9420211	A neutralizing antibody  that reacts with gp42 inhibits virus-cell fusion and blocks binding of  gp42 to HLA class II; antibody to HLA class II can inhibit infection,  and B cells that lack HLA class II can only be infected if HLA class II  expression is restored.	bind
46016	5	11357	6	NULL	NULL	0	NULL	HLA class II antibody	NULL		inhibits	NULL				infection	NULL				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_j-virol_72_1_9420211_s_4	9420211	A neutralizing antibody  that reacts with gp42 inhibits virus-cell fusion and blocks binding of  gp42 to HLA class II; antibody to HLA class II can inhibit infection,  and B cells that lack HLA class II can only be infected if HLA class II  expression is restored.	bind
46017	6	11357	6	NULL	NULL	0	NULL	B cells	NULL		lack	NULL				HLA class II	NULL				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_j-virol_72_1_9420211_s_4	9420211	A neutralizing antibody  that reacts with gp42 inhibits virus-cell fusion and blocks binding of  gp42 to HLA class II; antibody to HLA class II can inhibit infection,  and B cells that lack HLA class II can only be infected if HLA class II  expression is restored.	bind
46018	7	11357	6	10	NULL	0	NULL	statement 6	NULL		occurs upon 	NULL				HLA class II	NULL	restoration of ;;expression of			NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_j-virol_72_1_9420211_s_4	9420211	A neutralizing antibody  that reacts with gp42 inhibits virus-cell fusion and blocks binding of  gp42 to HLA class II; antibody to HLA class II can inhibit infection,  and B cells that lack HLA class II can only be infected if HLA class II  expression is restored.	bind
45536	1	11358	5	NULL	NULL	NULL	NULL	C-IIIJ1	GP		bind									regulatory element J	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_222_s_26	9012660	A new activity designated C-IIIJ1 binds to the regulatory element J, and a minor activity as well as HNF-4 binds to the regulatory element I. 5 8  Finally, the proximal apoA-IV promoter consists of four regulatory elements located between nucleotides -22 and -274.	bind
45537	2	11358	5	NULL	NULL	NULL	NULL	HNF-4	GP		bind									regulatory element I	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_222_s_26	9012660	A new activity designated C-IIIJ1 binds to the regulatory element J, and a minor activity as well as HNF-4 binds to the regulatory element I. 5 8  Finally, the proximal apoA-IV promoter consists of four regulatory elements located between nucleotides -22 and -274.	bind
45538	3	11358	5	NULL	NULL	NULL	NULL	apoA-IV	GP	proximal	consists of				promoter					regulatory elements between nucleotides -22 and -274	NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_222_s_26	9012660	A new activity designated C-IIIJ1 binds to the regulatory element J, and a minor activity as well as HNF-4 binds to the regulatory element I. 5 8  Finally, the proximal apoA-IV promoter consists of four regulatory elements located between nucleotides -22 and -274.	bind
46019	1	11358	6	NULL	NULL	0	NULL	C-IIIJ1	NULL		bind	NULL					NULL			regulatory element J	NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_222_s_26	9012660	A new activity designated C-IIIJ1 binds to the regulatory element J, and a minor activity as well as HNF-4 binds to the regulatory element I. 5 8  Finally, the proximal apoA-IV promoter consists of four regulatory elements located between nucleotides -22 and -274.	bind
46020	2	11358	6	NULL	NULL	0	NULL	HNF-4	NULL		bind	NULL					NULL			regulatory element I	NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_222_s_26	9012660	A new activity designated C-IIIJ1 binds to the regulatory element J, and a minor activity as well as HNF-4 binds to the regulatory element I. 5 8  Finally, the proximal apoA-IV promoter consists of four regulatory elements located between nucleotides -22 and -274.	bind
46021	3	11358	6	NULL	NULL	0	NULL	apoA-IV	NULL	proximal	consists of	NULL			promoter		NULL			regulatory elements between nucleotides -22 and -274	NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_1_222_s_26	9012660	A new activity designated C-IIIJ1 binds to the regulatory element J, and a minor activity as well as HNF-4 binds to the regulatory element I. 5 8  Finally, the proximal apoA-IV promoter consists of four regulatory elements located between nucleotides -22 and -274.	bind
45539	1	11359	5	NULL	NULL	NULL	NULL	Ry	Chemical		bind					RyR1	GP				NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_69_2_532_s_145	16249374	A new and somewhat unexpected finding was that unlike XeC, its hydroxylated derivative XeD (9-OH XeC;  Fig. 3B), and related structures ArC and 7-OH-XeA (data not shown) enhanced [3]Ry binding to RyR1 with an EC50 value of 10.6  plus-or-minus  1.1 muM ( n = 6) for XeD, 7.5  plus-or-minus  0.9 muM for ArC ( n = 4), and 11.4  plus-or-minus  0.8 muM for 7-OH-XeA ( n = 4).	bind
45540	2	11359	5	NULL	NULL	NULL	NULL	XeC	Chemical		does not enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_69_2_532_s_145	16249374	A new and somewhat unexpected finding was that unlike XeC, its hydroxylated derivative XeD (9-OH XeC;  Fig. 3B), and related structures ArC and 7-OH-XeA (data not shown) enhanced [3]Ry binding to RyR1 with an EC50 value of 10.6  plus-or-minus  1.1 muM ( n = 6) for XeD, 7.5  plus-or-minus  0.9 muM for ArC ( n = 4), and 11.4  plus-or-minus  0.8 muM for 7-OH-XeA ( n = 4).	bind
45541	3	11359	5	NULL	NULL	NULL	NULL	9-OH XeC	Chemical		is hydroxylated derivative of					XeD	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_69_2_532_s_145	16249374	A new and somewhat unexpected finding was that unlike XeC, its hydroxylated derivative XeD (9-OH XeC;  Fig. 3B), and related structures ArC and 7-OH-XeA (data not shown) enhanced [3]Ry binding to RyR1 with an EC50 value of 10.6  plus-or-minus  1.1 muM ( n = 6) for XeD, 7.5  plus-or-minus  0.9 muM for ArC ( n = 4), and 11.4  plus-or-minus  0.8 muM for 7-OH-XeA ( n = 4).	bind
45542	4	11359	5	NULL	NULL	NULL	NULL	9-OH XeC	Chemical		enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_69_2_532_s_145	16249374	A new and somewhat unexpected finding was that unlike XeC, its hydroxylated derivative XeD (9-OH XeC;  Fig. 3B), and related structures ArC and 7-OH-XeA (data not shown) enhanced [3]Ry binding to RyR1 with an EC50 value of 10.6  plus-or-minus  1.1 muM ( n = 6) for XeD, 7.5  plus-or-minus  0.9 muM for ArC ( n = 4), and 11.4  plus-or-minus  0.8 muM for 7-OH-XeA ( n = 4).	bind
45543	5	11359	5	NULL	NULL	NULL	NULL	ArC	Chemical		enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_69_2_532_s_145	16249374	A new and somewhat unexpected finding was that unlike XeC, its hydroxylated derivative XeD (9-OH XeC;  Fig. 3B), and related structures ArC and 7-OH-XeA (data not shown) enhanced [3]Ry binding to RyR1 with an EC50 value of 10.6  plus-or-minus  1.1 muM ( n = 6) for XeD, 7.5  plus-or-minus  0.9 muM for ArC ( n = 4), and 11.4  plus-or-minus  0.8 muM for 7-OH-XeA ( n = 4).	bind
45544	6	11359	5	NULL	NULL	NULL	NULL	7-OH-XeA	Chemical		enhance					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_69_2_532_s_145	16249374	A new and somewhat unexpected finding was that unlike XeC, its hydroxylated derivative XeD (9-OH XeC;  Fig. 3B), and related structures ArC and 7-OH-XeA (data not shown) enhanced [3]Ry binding to RyR1 with an EC50 value of 10.6  plus-or-minus  1.1 muM ( n = 6) for XeD, 7.5  plus-or-minus  0.9 muM for ArC ( n = 4), and 11.4  plus-or-minus  0.8 muM for 7-OH-XeA ( n = 4).	bind
46022	1	11359	6	NULL	NULL	0	NULL	Ry	NULL		bind	NULL				RyR1	NULL				NULL		0	NULL	NULL	NULL	gw70_molpharmacol_69_2_532_s_145	16249374	A new and somewhat unexpected finding was that unlike XeC, its hydroxylated derivative XeD (9-OH XeC;  Fig. 3B), and related structures ArC and 7-OH-XeA (data not shown) enhanced [3]Ry binding to RyR1 with an EC50 value of 10.6  plus-or-minus  1.1 muM ( n = 6) for XeD, 7.5  plus-or-minus  0.9 muM for ArC ( n = 4), and 11.4  plus-or-minus  0.8 muM for 7-OH-XeA ( n = 4).	bind
46023	2	11359	6	NULL	NULL	0	NULL	XeD	NULL		enhances	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molpharmacol_69_2_532_s_145	16249374	A new and somewhat unexpected finding was that unlike XeC, its hydroxylated derivative XeD (9-OH XeC;  Fig. 3B), and related structures ArC and 7-OH-XeA (data not shown) enhanced [3]Ry binding to RyR1 with an EC50 value of 10.6  plus-or-minus  1.1 muM ( n = 6) for XeD, 7.5  plus-or-minus  0.9 muM for ArC ( n = 4), and 11.4  plus-or-minus  0.8 muM for 7-OH-XeA ( n = 4).	bind
46024	3	11359	6	NULL	NULL	0	NULL	7-OH-XeA	NULL		enhances	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molpharmacol_69_2_532_s_145	16249374	A new and somewhat unexpected finding was that unlike XeC, its hydroxylated derivative XeD (9-OH XeC;  Fig. 3B), and related structures ArC and 7-OH-XeA (data not shown) enhanced [3]Ry binding to RyR1 with an EC50 value of 10.6  plus-or-minus  1.1 muM ( n = 6) for XeD, 7.5  plus-or-minus  0.9 muM for ArC ( n = 4), and 11.4  plus-or-minus  0.8 muM for 7-OH-XeA ( n = 4).	bind
46025	4	11359	6	NULL	NULL	0	NULL	XeC	NULL		does not enhance	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molpharmacol_69_2_532_s_145	16249374	A new and somewhat unexpected finding was that unlike XeC, its hydroxylated derivative XeD (9-OH XeC;  Fig. 3B), and related structures ArC and 7-OH-XeA (data not shown) enhanced [3]Ry binding to RyR1 with an EC50 value of 10.6  plus-or-minus  1.1 muM ( n = 6) for XeD, 7.5  plus-or-minus  0.9 muM for ArC ( n = 4), and 11.4  plus-or-minus  0.8 muM for 7-OH-XeA ( n = 4).	bind
51502	5	11359	6	10	NULL	0	NULL	ArC	NULL		enhance	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molpharmacol_69_2_532_s_145	16249374	A new and somewhat unexpected finding was that unlike XeC, its hydroxylated derivative XeD (9-OH XeC;  Fig. 3B), and related structures ArC and 7-OH-XeA (data not shown) enhanced [3]Ry binding to RyR1 with an EC50 value of 10.6  plus-or-minus  1.1 muM ( n = 6) for XeD, 7.5  plus-or-minus  0.9 muM for ArC ( n = 4), and 11.4  plus-or-minus  0.8 muM for 7-OH-XeA ( n = 4).	bind
51503	6	11359	6	10	NULL	0	NULL	9-OH XeC			is hydroxylated derivative of					XeD					NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_69_2_532_s_145	16249374	A new and somewhat unexpected finding was that unlike XeC, its hydroxylated derivative XeD (9-OH XeC;  Fig. 3B), and related structures ArC and 7-OH-XeA (data not shown) enhanced [3]Ry binding to RyR1 with an EC50 value of 10.6  plus-or-minus  1.1 muM ( n = 6) for XeD, 7.5  plus-or-minus  0.9 muM for ArC ( n = 4), and 11.4  plus-or-minus  0.8 muM for 7-OH-XeA ( n = 4).	bind
45545	1	11361	5	NULL	NULL	NULL	NULL	ATP	Chemical		bind					Ala	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_21_4134_s_225	15470502	A new ATP-binding mutant was constructed replacing Asn33 that chelates  Mg2+ and is essential for ATP binding with Ala ( Figure 3B).	bind
45546	2	11361	5	NULL	NULL	NULL	NULL	ATP-binding mutant \t	GP		chelates					Mg2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_21_4134_s_225	15470502	A new ATP-binding mutant was constructed replacing Asn33 that chelates  Mg2+ and is essential for ATP binding with Ala ( Figure 3B).	bind
45547	3	11361	5	NULL	NULL	NULL	NULL	Asn33	AminoAcid		is replaced in					ATP-binding mutant	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_21_4134_s_225	15470502	A new ATP-binding mutant was constructed replacing Asn33 that chelates  Mg2+ and is essential for ATP binding with Ala ( Figure 3B).	bind
45548	4	11361	5	NULL	NULL	NULL	NULL	statement 3	Process		is essential for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_21_4134_s_225	15470502	A new ATP-binding mutant was constructed replacing Asn33 that chelates  Mg2+ and is essential for ATP binding with Ala ( Figure 3B).	bind
46026	1	11361	6	10	NULL	0	NULL	ATP			bind					Ala					NULL		NULL	NULL	NULL	NULL	gw70_embo_23_21_4134_s_225	15470502	A new ATP-binding mutant was constructed replacing Asn33 that chelates  Mg2+ and is essential for ATP binding with Ala ( Figure 3B).	bind
46027	2	11361	6	NULL	NULL	0	NULL	ATP-binding mutant	NULL		is essential for	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_23_21_4134_s_225	15470502	A new ATP-binding mutant was constructed replacing Asn33 that chelates  Mg2+ and is essential for ATP binding with Ala ( Figure 3B).	bind
46028	3	11361	6	NULL	NULL	0	NULL	ATP-binding mutant	NULL		chelates	NULL				Mg2+	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_23_21_4134_s_225	15470502	A new ATP-binding mutant was constructed replacing Asn33 that chelates  Mg2+ and is essential for ATP binding with Ala ( Figure 3B).	bind
51504	4	11361	6	10	NULL	0	NULL	Asn33	NULL		is replaced in	NULL				ATP-binding mutant	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_23_21_4134_s_225	15470502	A new ATP-binding mutant was constructed replacing Asn33 that chelates  Mg2+ and is essential for ATP binding with Ala ( Figure 3B).	bind
45549	1	11362	5	NULL	NULL	NULL	NULL	GLYT-1	GP		is a type of					glycine transporter	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_6128_s_22	12431995	A new C-terminal splice variant of the glycine transporter GLYT-1 bound to rho1 ( ), while the microtubule-associated protein 1B (MAP-1B) interacted with rho1 and rho2 and was co-localized with GABAC receptors in the retina ( ).	bind
45550	2	11362	5	NULL	NULL	NULL	NULL	GLYT-1	GP	splice variant of	bind			C-terminal		rho1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_6128_s_22	12431995	A new C-terminal splice variant of the glycine transporter GLYT-1 bound to rho1 ( ), while the microtubule-associated protein 1B (MAP-1B) interacted with rho1 and rho2 and was co-localized with GABAC receptors in the retina ( ).	bind
45551	3	11362	5	NULL	NULL	NULL	NULL	MAP-1B	GP		is					microtubule-associated protein 1B	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_6128_s_22	12431995	A new C-terminal splice variant of the glycine transporter GLYT-1 bound to rho1 ( ), while the microtubule-associated protein 1B (MAP-1B) interacted with rho1 and rho2 and was co-localized with GABAC receptors in the retina ( ).	bind
45552	4	11362	5	NULL	NULL	NULL	NULL	MAP-1B	GP		interacts with					rho1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_6128_s_22	12431995	A new C-terminal splice variant of the glycine transporter GLYT-1 bound to rho1 ( ), while the microtubule-associated protein 1B (MAP-1B) interacted with rho1 and rho2 and was co-localized with GABAC receptors in the retina ( ).	bind
45553	5	11362	5	NULL	NULL	NULL	NULL	MAP-1B	GP		interacts with					rho2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_6128_s_22	12431995	A new C-terminal splice variant of the glycine transporter GLYT-1 bound to rho1 ( ), while the microtubule-associated protein 1B (MAP-1B) interacted with rho1 and rho2 and was co-localized with GABAC receptors in the retina ( ).	bind
45554	6	11362	5	NULL	NULL	NULL	NULL	MAP-1B	GP		co-localizes with					GABAC receptors	GP				NULL	retina	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_6128_s_22	12431995	A new C-terminal splice variant of the glycine transporter GLYT-1 bound to rho1 ( ), while the microtubule-associated protein 1B (MAP-1B) interacted with rho1 and rho2 and was co-localized with GABAC receptors in the retina ( ).	bind
46029	1	11362	6	NULL	NULL	0	NULL	GLYT-1	NULL	splice variant	bind	NULL		C-terminal		rho1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_8_6128_s_22	12431995	A new C-terminal splice variant of the glycine transporter GLYT-1 bound to rho1 ( ), while the microtubule-associated protein 1B (MAP-1B) interacted with rho1 and rho2 and was co-localized with GABAC receptors in the retina ( ).	bind
46030	2	11362	6	10	NULL	0	NULL	MAP-1B			interacts with					rho1					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_6128_s_22	12431995	A new C-terminal splice variant of the glycine transporter GLYT-1 bound to rho1 ( ), while the microtubule-associated protein 1B (MAP-1B) interacted with rho1 and rho2 and was co-localized with GABAC receptors in the retina ( ).	bind
46031	3	11362	6	NULL	NULL	0	NULL	MAP-1B	NULL		interacts with	NULL				rho2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_8_6128_s_22	12431995	A new C-terminal splice variant of the glycine transporter GLYT-1 bound to rho1 ( ), while the microtubule-associated protein 1B (MAP-1B) interacted with rho1 and rho2 and was co-localized with GABAC receptors in the retina ( ).	bind
46032	4	11362	6	NULL	NULL	0	NULL	MAP-1B	NULL		is	NULL				microtubule-associated protein 1B	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_8_6128_s_22	12431995	A new C-terminal splice variant of the glycine transporter GLYT-1 bound to rho1 ( ), while the microtubule-associated protein 1B (MAP-1B) interacted with rho1 and rho2 and was co-localized with GABAC receptors in the retina ( ).	bind
46033	5	11362	6	10	NULL	0	NULL	MAP-1B	NULL		co-localized with	NULL				GABAC receptors	NULL				NULL	retina	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_6128_s_22	12431995	A new C-terminal splice variant of the glycine transporter GLYT-1 bound to rho1 ( ), while the microtubule-associated protein 1B (MAP-1B) interacted with rho1 and rho2 and was co-localized with GABAC receptors in the retina ( ).	bind
46034	6	11362	6	10	NULL	0	NULL	GLYT-1	NULL		is a type of	NULL				glycine transporter	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_8_6128_s_22	12431995	A new C-terminal splice variant of the glycine transporter GLYT-1 bound to rho1 ( ), while the microtubule-associated protein 1B (MAP-1B) interacted with rho1 and rho2 and was co-localized with GABAC receptors in the retina ( ).	bind
45555	1	11364	5	NULL	NULL	NULL	NULL	PR inhibitors	Chemical	symmetric	bind					HIV PR	GP				NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_64_4_725_s_147	11104817	A new direction was thus taken when it appeared that symmetric PR inhibitors could bind the HIV PR in an asymmetric fashion ( ,  ,  ).	bind
51505	2	11364	5	NULL	NULL	NULL	NULL	statement 1	Process		occurs in a					asymmetric fashion					NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_64_4_725_s_147	11104817	A new direction was thus taken when it appeared that symmetric PR inhibitors could bind the HIV PR in an asymmetric fashion ( ,  ,  ).	bind
46038	1	11364	6	10	NULL	0	NULL	PR inhibitors		symmetric	bind					HIV PR					NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_64_4_725_s_147	11104817	A new direction was thus taken when it appeared that symmetric PR inhibitors could bind the HIV PR in an asymmetric fashion ( ,  ,  ).	bind
46039	2	11364	6	NULL	NULL	0	NULL	statement 1	NULL		occurs in an	NULL				asymmetric fashion	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_64_4_725_s_147	11104817	A new direction was thus taken when it appeared that symmetric PR inhibitors could bind the HIV PR in an asymmetric fashion ( ,  ,  ).	bind
45556	1	11366	5	NULL	NULL	NULL	NULL	W600	Chemical		is					water molecule	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_24_16669_s_65	10358003	A new feature of the active site is a highly ordered (B = 21.9 Ang 2) water molecule (W600) bound to the O1G oxygen of the gamma-phosphate (Fig.  1 and Fig.  2 A).	bind
45557	2	11366	5	NULL	NULL	NULL	NULL	W600	Chemical		bind					O1G oxygen	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_24_16669_s_65	10358003	A new feature of the active site is a highly ordered (B = 21.9 Ang 2) water molecule (W600) bound to the O1G oxygen of the gamma-phosphate (Fig.  1 and Fig.  2 A).	bind
45558	3	11366	5	NULL	NULL	NULL	NULL	O1G oxygen	Chemical		is present in					gamma-phosphate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_24_16669_s_65	10358003	A new feature of the active site is a highly ordered (B = 21.9 Ang 2) water molecule (W600) bound to the O1G oxygen of the gamma-phosphate (Fig.  1 and Fig.  2 A).	bind
46040	1	11366	6	10	NULL	0	NULL	W600	NULL		bind	NULL				gamma-phosphate	NULL		O1G oxygen		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_24_16669_s_65	10358003	A new feature of the active site is a highly ordered (B = 21.9 Ang 2) water molecule (W600) bound to the O1G oxygen of the gamma-phosphate (Fig.  1 and Fig.  2 A).	bind
51506	2	11366	6	10	NULL	0	NULL	W600	NULL		is	NULL				water molecule	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_24_16669_s_65	10358003	A new feature of the active site is a highly ordered (B = 21.9 Ang 2) water molecule (W600) bound to the O1G oxygen of the gamma-phosphate (Fig.  1 and Fig.  2 A).	bind
45666	1	11370	5	NULL	NULL	NULL	NULL	O2	Chemical		bind		rapidly;;high affinity			heme	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_24_14100_s_144	9826660	A new round of catalysis then is initiated by O2 binding to heme (Eq.   3), which has been shown to occur very rapidly and with high affinity ( 27).	bind
45667	2	11370	5	NULL	NULL	NULL	NULL	statement 1	Process		initiates					catalysis	Process	new round of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_24_14100_s_144	9826660	A new round of catalysis then is initiated by O2 binding to heme (Eq.   3), which has been shown to occur very rapidly and with high affinity ( 27).	bind
46041	1	11370	6	10	NULL	0	NULL	O2	NULL		bind	NULL	rapidly;; high affinity			heme	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_24_14100_s_144	9826660	A new round of catalysis then is initiated by O2 binding to heme (Eq.   3), which has been shown to occur very rapidly and with high affinity ( 27).	bind
46042	2	11370	6	NULL	NULL	0	NULL	statement 1	NULL		initiates	NULL				catalysis	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_24_14100_s_144	9826660	A new round of catalysis then is initiated by O2 binding to heme (Eq.   3), which has been shown to occur very rapidly and with high affinity ( 27).	bind
45668	1	11371	5	NULL	NULL	NULL	NULL	colchicine	Chemical		bind					tubulin	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-med-chem_49_13_16789746_s_2	16789746	A new series of compounds in which the 2-amino-5-chlorophenyl ring of phenstatin  analogue 7 was replaced with a 2-amino-5-aryl thiophene was synthesized  and evaluated for antiproliferative activity and for inhibition of tubulin  polymerization and colchicine binding to tubulin.	bind
46043	1	11371	6	NULL	NULL	0	NULL	colchicine	NULL		bind	NULL				tubulin	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-med-chem_49_13_16789746_s_2	16789746	A new series of compounds in which the 2-amino-5-chlorophenyl ring of phenstatin  analogue 7 was replaced with a 2-amino-5-aryl thiophene was synthesized  and evaluated for antiproliferative activity and for inhibition of tubulin  polymerization and colchicine binding to tubulin.	bind
45669	1	11372	5	NULL	NULL	NULL	NULL	Nhp6	GP		bind					Gal4p	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_25_13732_s_143	11095729	A New Split-Ub-Based Screen Identifies Nhp6 as a Binding Partner of Gal4p and Tup1p.	bind
45670	2	11372	5	NULL	NULL	NULL	NULL	Nhp6	GP		bind					Tup1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_25_13732_s_143	11095729	A New Split-Ub-Based Screen Identifies Nhp6 as a Binding Partner of Gal4p and Tup1p.	bind
46044	1	11372	6	NULL	NULL	0	NULL	Nhp6	NULL		bind	NULL				Gal4p	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_25_13732_s_143	11095729	A New Split-Ub-Based Screen Identifies Nhp6 as a Binding Partner of Gal4p and Tup1p.	bind
46045	2	11372	6	NULL	NULL	0	NULL	Nhp6	NULL		bind	NULL				Tup1p	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_25_13732_s_143	11095729	A New Split-Ub-Based Screen Identifies Nhp6 as a Binding Partner of Gal4p and Tup1p.	bind
45671	1	11373	5	NULL	NULL	NULL	NULL				bind		specifically	cohesin domain		CipA	GP	Clostridium thermocellum	dockerin domain		NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_3_703_s_389	12533446	A new type of cohesin domain that specifically binds the dockerin domain of the  Clostridium thermocellum cellulosome integrating protein CipA.	bind
45672	2	11373	5	NULL	NULL	NULL	NULL	CipA	GP		is					cellulosome integrating protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_3_703_s_389	12533446	A new type of cohesin domain that specifically binds the dockerin domain of the  Clostridium thermocellum cellulosome integrating protein CipA.	bind
46046	1	11373	6	NULL	NULL	0	NULL	CipA	NULL	Clostridium thermocellum	bind	NULL	specifically	dockerin domain			NULL		cohesin domain		NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_3_703_s_389	12533446	A new type of cohesin domain that specifically binds the dockerin domain of the  Clostridium thermocellum cellulosome integrating protein CipA.	bind
46047	2	11373	6	10	NULL	0	NULL	CipA	NULL		is	NULL				cellulosome integrating protein	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_185_3_703_s_389	12533446	A new type of cohesin domain that specifically binds the dockerin domain of the  Clostridium thermocellum cellulosome integrating protein CipA.	bind
45673	1	11375	5	NULL	NULL	NULL	NULL	laccase	GP		bind					Ag surface	Chemical	thiol-coated			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_appl-spectrosc_60_7_16854262_s_3	16854262	A new, indirect way of monitoring laccase  bound to the thiol-coated Ag and Au surfaces is presented.	bind
45674	2	11375	5	NULL	NULL	NULL	NULL	laccase	GP		bind					Au surface	Chemical	thiol-coated			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_appl-spectrosc_60_7_16854262_s_3	16854262	A new, indirect way of monitoring laccase  bound to the thiol-coated Ag and Au surfaces is presented.	bind
46048	1	11375	6	NULL	NULL	0	NULL	laccase	NULL		bind	NULL				Ag surface	NULL	thiol-coated			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_appl-spectrosc_60_7_16854262_s_3	16854262	A new, indirect way of monitoring laccase  bound to the thiol-coated Ag and Au surfaces is presented.	bind
46049	2	11375	6	NULL	NULL	0	NULL	laccase	NULL		bind	NULL				Au surface	NULL	thiol-coated			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_appl-spectrosc_60_7_16854262_s_3	16854262	A new, indirect way of monitoring laccase  bound to the thiol-coated Ag and Au surfaces is presented.	bind
45675	1	11376	5	NULL	NULL	NULL	NULL	hGli2	GP		bind									TRE-2	NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_19_0_475_s_92	11244044	A newly identified protein, hGli2, binds to TRE-2 ( 51), and the binding of hGli2 to TRE-2 is essential for Tax-mediated  trans-activation of one copy of the 21-bp enhancer.	bind
45676	2	11376	5	NULL	NULL	NULL	NULL	Tax	GP		mediates							trans-activation of		21-bp enhancer	NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_19_0_475_s_92	11244044	A newly identified protein, hGli2, binds to TRE-2 ( 51), and the binding of hGli2 to TRE-2 is essential for Tax-mediated  trans-activation of one copy of the 21-bp enhancer.	bind
45678	3	11376	5	NULL	NULL	NULL	NULL	statement 1	Process		is essential for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_19_0_475_s_92	11244044	A newly identified protein, hGli2, binds to TRE-2 ( 51), and the binding of hGli2 to TRE-2 is essential for Tax-mediated  trans-activation of one copy of the 21-bp enhancer.	bind
46050	1	11376	6	10	NULL	0	NULL	hGli2	NULL		bind	NULL					NULL			TRE-2	NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_19_0_475_s_92	11244044	A newly identified protein, hGli2, binds to TRE-2 ( 51), and the binding of hGli2 to TRE-2 is essential for Tax-mediated  trans-activation of one copy of the 21-bp enhancer.	bind
46051	2	11376	6	10	NULL	0	NULL	Tax	NULL		mediates	NULL					NULL	transactivation of		21-bp enhancer	NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_19_0_475_s_92	11244044	A newly identified protein, hGli2, binds to TRE-2 ( 51), and the binding of hGli2 to TRE-2 is essential for Tax-mediated  trans-activation of one copy of the 21-bp enhancer.	bind
46052	3	11376	6	NULL	NULL	0	NULL	statement 1	NULL		is essential for	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_19_0_475_s_92	11244044	A newly identified protein, hGli2, binds to TRE-2 ( 51), and the binding of hGli2 to TRE-2 is essential for Tax-mediated  trans-activation of one copy of the 21-bp enhancer.	bind
45680	1	11377	5	NULL	NULL	NULL	NULL	ACA	GP		is					agglutinin	GP	Amaranthus caudatus 			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_cancer-res_51_2_1985783_s_2	1985783	A newly isolated lectin, Amaranthus caudatus agglutinin (also called amaranthin  or ACA), which binds to the Thomsen-Friedenreich antigen (T-antigen) and  its sialylated variants, was used as a histochemical probe for proliferating  cells in sections of human colonic tissues.	bind
45681	2	11377	5	NULL	NULL	NULL	NULL	ACA	GP		is a type of					lectin	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_cancer-res_51_2_1985783_s_2	1985783	A newly isolated lectin, Amaranthus caudatus agglutinin (also called amaranthin  or ACA), which binds to the Thomsen-Friedenreich antigen (T-antigen) and  its sialylated variants, was used as a histochemical probe for proliferating  cells in sections of human colonic tissues.	bind
45682	3	11377	5	NULL	NULL	NULL	NULL	amaranthin	GP		is a synonym of					ACA	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_cancer-res_51_2_1985783_s_2	1985783	A newly isolated lectin, Amaranthus caudatus agglutinin (also called amaranthin  or ACA), which binds to the Thomsen-Friedenreich antigen (T-antigen) and  its sialylated variants, was used as a histochemical probe for proliferating  cells in sections of human colonic tissues.	bind
45683	4	11377	5	NULL	NULL	NULL	NULL	ACA	GP		bind					Thomsen-Friedenreich antigen	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_cancer-res_51_2_1985783_s_2	1985783	A newly isolated lectin, Amaranthus caudatus agglutinin (also called amaranthin  or ACA), which binds to the Thomsen-Friedenreich antigen (T-antigen) and  its sialylated variants, was used as a histochemical probe for proliferating  cells in sections of human colonic tissues.	bind
45684	5	11377	5	NULL	NULL	NULL	NULL	Thomsen-Friedenreich antigen	GP		is					T-antigen	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_cancer-res_51_2_1985783_s_2	1985783	A newly isolated lectin, Amaranthus caudatus agglutinin (also called amaranthin  or ACA), which binds to the Thomsen-Friedenreich antigen (T-antigen) and  its sialylated variants, was used as a histochemical probe for proliferating  cells in sections of human colonic tissues.	bind
45685	6	11377	5	NULL	NULL	NULL	NULL	ACA	GP		bind					Thomsen-Friedenreich antigen	GP	sialylated variants of			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_cancer-res_51_2_1985783_s_2	1985783	A newly isolated lectin, Amaranthus caudatus agglutinin (also called amaranthin  or ACA), which binds to the Thomsen-Friedenreich antigen (T-antigen) and  its sialylated variants, was used as a histochemical probe for proliferating  cells in sections of human colonic tissues.	bind
46117	1	11377	6	NULL	NULL	0	NULL	agglutinin	NULL		is	NULL				amaranthin	NULL				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_cancer-res_51_2_1985783_s_2	1985783	A newly isolated lectin, Amaranthus caudatus agglutinin (also called amaranthin  or ACA), which binds to the Thomsen-Friedenreich antigen (T-antigen) and  its sialylated variants, was used as a histochemical probe for proliferating  cells in sections of human colonic tissues.	bind
46118	2	11377	6	NULL	NULL	0	NULL	agglutinin	NULL		is	NULL				ACA	NULL				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_cancer-res_51_2_1985783_s_2	1985783	A newly isolated lectin, Amaranthus caudatus agglutinin (also called amaranthin  or ACA), which binds to the Thomsen-Friedenreich antigen (T-antigen) and  its sialylated variants, was used as a histochemical probe for proliferating  cells in sections of human colonic tissues.	bind
46119	3	11377	6	NULL	NULL	0	NULL	agglutinin	NULL		is a type of	NULL				lectin	NULL				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_cancer-res_51_2_1985783_s_2	1985783	A newly isolated lectin, Amaranthus caudatus agglutinin (also called amaranthin  or ACA), which binds to the Thomsen-Friedenreich antigen (T-antigen) and  its sialylated variants, was used as a histochemical probe for proliferating  cells in sections of human colonic tissues.	bind
46120	4	11377	6	NULL	NULL	0	NULL	agglutinin	NULL	Amaranthus caudatus	bind	NULL				T-antigen	NULL				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_cancer-res_51_2_1985783_s_2	1985783	A newly isolated lectin, Amaranthus caudatus agglutinin (also called amaranthin  or ACA), which binds to the Thomsen-Friedenreich antigen (T-antigen) and  its sialylated variants, was used as a histochemical probe for proliferating  cells in sections of human colonic tissues.	bind
46121	5	11377	6	NULL	NULL	0	NULL	T-antigen	NULL		is	NULL				Thomsen-Friedenreich antigen	NULL				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_cancer-res_51_2_1985783_s_2	1985783	A newly isolated lectin, Amaranthus caudatus agglutinin (also called amaranthin  or ACA), which binds to the Thomsen-Friedenreich antigen (T-antigen) and  its sialylated variants, was used as a histochemical probe for proliferating  cells in sections of human colonic tissues.	bind
46122	6	11377	6	NULL	NULL	0	NULL	agglutinin	NULL	Amaranthus caudatus	bind	NULL				T-antigen	NULL	sialyated			NULL		0	NULL	NULL	NULL	abs-batch0517-0529_cancer-res_51_2_1985783_s_2	1985783	A newly isolated lectin, Amaranthus caudatus agglutinin (also called amaranthin  or ACA), which binds to the Thomsen-Friedenreich antigen (T-antigen) and  its sialylated variants, was used as a histochemical probe for proliferating  cells in sections of human colonic tissues.	bind
45686	1	11380	5	NULL	NULL	NULL	NULL	RSK2	GP		is a type of					Ras-dependent protein kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_429_3_254_s_114	9662427	A NGF-inducible, Ras-dependent protein kinase, which was identified as RSK2, and catalyzes the phosphorylation of CREB (the cyclic AMP response element binding protein), was found to trigger this activation [ 22,   23].	bind
45687	2	11380	5	NULL	NULL	NULL	NULL	NGF	GP		induces					RSK2	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_429_3_254_s_114	9662427	A NGF-inducible, Ras-dependent protein kinase, which was identified as RSK2, and catalyzes the phosphorylation of CREB (the cyclic AMP response element binding protein), was found to trigger this activation [ 22,   23].	bind
45688	3	11380	5	NULL	NULL	NULL	NULL	RSK2	GP		catalyzes					CREB	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw60_febslett_429_3_254_s_114	9662427	A NGF-inducible, Ras-dependent protein kinase, which was identified as RSK2, and catalyzes the phosphorylation of CREB (the cyclic AMP response element binding protein), was found to trigger this activation [ 22,   23].	bind
45689	4	11380	5	NULL	NULL	NULL	NULL	CREB	GP		is					cyclic AMP response element binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_429_3_254_s_114	9662427	A NGF-inducible, Ras-dependent protein kinase, which was identified as RSK2, and catalyzes the phosphorylation of CREB (the cyclic AMP response element binding protein), was found to trigger this activation [ 22,   23].	bind
46053	1	11380	6	NULL	NULL	0	NULL	RSK2	NULL		catalyzes	NULL				CREB	NULL	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_febslett_429_3_254_s_114	9662427	A NGF-inducible, Ras-dependent protein kinase, which was identified as RSK2, and catalyzes the phosphorylation of CREB (the cyclic AMP response element binding protein), was found to trigger this activation [ 22,   23].	bind
46054	2	11380	6	NULL	NULL	0	NULL	RSK2	NULL		is a type of	NULL				Ras-dependent protein kinase	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_429_3_254_s_114	9662427	A NGF-inducible, Ras-dependent protein kinase, which was identified as RSK2, and catalyzes the phosphorylation of CREB (the cyclic AMP response element binding protein), was found to trigger this activation [ 22,   23].	bind
46055	3	11380	6	NULL	NULL	0	NULL	NGF	NULL		induces	NULL				RSK2	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_429_3_254_s_114	9662427	A NGF-inducible, Ras-dependent protein kinase, which was identified as RSK2, and catalyzes the phosphorylation of CREB (the cyclic AMP response element binding protein), was found to trigger this activation [ 22,   23].	bind
46056	4	11380	6	NULL	NULL	0	NULL	CREB	NULL		is	NULL				cyclic AMP response element binding protein	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_429_3_254_s_114	9662427	A NGF-inducible, Ras-dependent protein kinase, which was identified as RSK2, and catalyzes the phosphorylation of CREB (the cyclic AMP response element binding protein), was found to trigger this activation [ 22,   23].	bind
45690	1	11381	5	NULL	NULL	NULL	NULL	junction peptide	AminoAcid	nonself	comprises of					ETV6 and AML1 	GP	residues of			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_2_455_s_211	9664088	A nine  amino acid-long, nonself, junction peptide comprising four  ETV6 and five AML1 residues binds to HLA-A2.1 molecules  and induces in vitro CTL responses from both HLA-A2.1+  healthy donors and ALL-patients.	bind
45691	2	11381	5	NULL	NULL	NULL	NULL	statement 1			bind					HLA-A2.1 molecules	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_2_455_s_211	9664088	A nine  amino acid-long, nonself, junction peptide comprising four  ETV6 and five AML1 residues binds to HLA-A2.1 molecules  and induces in vitro CTL responses from both HLA-A2.1+  healthy donors and ALL-patients.	bind
45692	3	11381	5	NULL	NULL	NULL	NULL	statement 2	Process		induces					CTL responses	Process				NULL	in vitro in HLA-A2.1+ healthy donors	NULL	NULL	NULL	NULL	gw60_jclininvest_102_2_455_s_211	9664088	A nine  amino acid-long, nonself, junction peptide comprising four  ETV6 and five AML1 residues binds to HLA-A2.1 molecules  and induces in vitro CTL responses from both HLA-A2.1+  healthy donors and ALL-patients.	bind
45693	4	11381	5	NULL	NULL	NULL	NULL	statement 2	Process		induces					CTL responses	Process				NULL	in vitro in ALL-patients	NULL	NULL	NULL	NULL	gw60_jclininvest_102_2_455_s_211	9664088	A nine  amino acid-long, nonself, junction peptide comprising four  ETV6 and five AML1 residues binds to HLA-A2.1 molecules  and induces in vitro CTL responses from both HLA-A2.1+  healthy donors and ALL-patients.	bind
46127	1	11381	6	10	NULL	0	NULL	peptide			comprises of					 ETV6 and AML1		residues of			NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_102_2_455_s_211	9664088	A nine  amino acid-long, nonself, junction peptide comprising four  ETV6 and five AML1 residues binds to HLA-A2.1 molecules  and induces in vitro CTL responses from both HLA-A2.1+  healthy donors and ALL-patients.	bind
46128	2	11381	6	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL				HLA-A2.1 molecules	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_102_2_455_s_211	9664088	A nine  amino acid-long, nonself, junction peptide comprising four  ETV6 and five AML1 residues binds to HLA-A2.1 molecules  and induces in vitro CTL responses from both HLA-A2.1+  healthy donors and ALL-patients.	bind
46129	3	11381	6	10	NULL	0	NULL	statement 2	NULL		induces	NULL				CTL responses	NULL				NULL	in vitro in HLA-A2.1+ healthy donors	NULL	NULL	NULL	NULL	gw60_jclininvest_102_2_455_s_211	9664088	A nine  amino acid-long, nonself, junction peptide comprising four  ETV6 and five AML1 residues binds to HLA-A2.1 molecules  and induces in vitro CTL responses from both HLA-A2.1+  healthy donors and ALL-patients.	bind
46130	4	11381	6	10	NULL	0	NULL	statement 2	NULL		induces	NULL				CTL responses	NULL				NULL	invitro in ALL-patients	NULL	NULL	NULL	NULL	gw60_jclininvest_102_2_455_s_211	9664088	A nine  amino acid-long, nonself, junction peptide comprising four  ETV6 and five AML1 residues binds to HLA-A2.1 molecules  and induces in vitro CTL responses from both HLA-A2.1+  healthy donors and ALL-patients.	bind
45694	2	11382	5	NULL	NULL	NULL	NULL	statement 1	AminoAcid		bind		strongly			HLA-A2 antigen	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_clin-cancer-res_7_11_11705846_s_4	11705846	A nine-amino acid peptide  derived from hTERT binds strongly to HLA-A2 antigen and elicits CTL responses  against a broad panel of hTERT+ tumors (but not hTERT+ hematopoietic progenitor  cells).	bind
45695	3	11382	5	NULL	NULL	NULL	NULL	statement 2	Process		elicits					CTL responses	Process				NULL	hTERT+ tumors	NULL	NULL	NULL	NULL	abs-batch0650-0679_clin-cancer-res_7_11_11705846_s_4	11705846	A nine-amino acid peptide  derived from hTERT binds strongly to HLA-A2 antigen and elicits CTL responses  against a broad panel of hTERT+ tumors (but not hTERT+ hematopoietic progenitor  cells).	bind
45696	4	11382	5	NULL	NULL	NULL	NULL	statement 2	Process		does not elicit					CTL responses	Process				NULL	hTERT+ hematopoietic progenitor cells	NULL	NULL	NULL	NULL	abs-batch0650-0679_clin-cancer-res_7_11_11705846_s_4	11705846	A nine-amino acid peptide  derived from hTERT binds strongly to HLA-A2 antigen and elicits CTL responses  against a broad panel of hTERT+ tumors (but not hTERT+ hematopoietic progenitor  cells).	bind
51508	1	11382	5	NULL	NULL	NULL	NULL	nine-amino acid peptide	AminoAcid		derived from					hTERT	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_clin-cancer-res_7_11_11705846_s_4	11705846	A nine-amino acid peptide  derived from hTERT binds strongly to HLA-A2 antigen and elicits CTL responses  against a broad panel of hTERT+ tumors (but not hTERT+ hematopoietic progenitor  cells).	bind
46057	1	11382	6	NULL	NULL	0	NULL	nine-amino acid peptide	NULL		is derived from	NULL				hTERT	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_clin-cancer-res_7_11_11705846_s_4	11705846	A nine-amino acid peptide  derived from hTERT binds strongly to HLA-A2 antigen and elicits CTL responses  against a broad panel of hTERT+ tumors (but not hTERT+ hematopoietic progenitor  cells).	bind
46058	2	11382	6	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL	strongly			HLA-A2 antigen	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_clin-cancer-res_7_11_11705846_s_4	11705846	A nine-amino acid peptide  derived from hTERT binds strongly to HLA-A2 antigen and elicits CTL responses  against a broad panel of hTERT+ tumors (but not hTERT+ hematopoietic progenitor  cells).	bind
46059	3	11382	6	10	NULL	0	NULL	statement 2	NULL		elicits	NULL				CTL responses	NULL				NULL	hTERT+ tumors	NULL	NULL	NULL	NULL	abs-batch0650-0679_clin-cancer-res_7_11_11705846_s_4	11705846	A nine-amino acid peptide  derived from hTERT binds strongly to HLA-A2 antigen and elicits CTL responses  against a broad panel of hTERT+ tumors (but not hTERT+ hematopoietic progenitor  cells).	bind
46060	4	11382	6	10	NULL	0	NULL	statement 2	NULL		does not elicit	NULL				CTL responses	NULL				NULL	hTERT+ hematopoietic progenitor cells	NULL	NULL	NULL	NULL	abs-batch0650-0679_clin-cancer-res_7_11_11705846_s_4	11705846	A nine-amino acid peptide  derived from hTERT binds strongly to HLA-A2 antigen and elicits CTL responses  against a broad panel of hTERT+ tumors (but not hTERT+ hematopoietic progenitor  cells).	bind
45697	1	11383	5	NULL	NULL	NULL	NULL	collagen	GP		bind					alpha2	GP		I-domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_44_31493_s_36	10531352	A nine-residue aspartate-containing peptide was obtained from the metalloproteinase that, when cyclized through the addition of terminal cysteines and oxidized to form a disulfide bond, was found to inhibit collagen binding to the alpha2 I-domain.	bind
45698	2	11383	5	NULL	NULL	NULL	NULL	aspartate-containing peptide	AminoAcid		is obtained from					metalloproteinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_44_31493_s_36	10531352	A nine-residue aspartate-containing peptide was obtained from the metalloproteinase that, when cyclized through the addition of terminal cysteines and oxidized to form a disulfide bond, was found to inhibit collagen binding to the alpha2 I-domain.	bind
45699	3	11383	5	NULL	NULL	NULL	NULL	statement 2	AminoAcid		is cyclized through					cysteines	AminoAcid	addition of;;terminal			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_44_31493_s_36	10531352	A nine-residue aspartate-containing peptide was obtained from the metalloproteinase that, when cyclized through the addition of terminal cysteines and oxidized to form a disulfide bond, was found to inhibit collagen binding to the alpha2 I-domain.	bind
45700	4	11383	5	NULL	NULL	NULL	NULL	statement 3	AminoAcid		undergoes					oxidation	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_44_31493_s_36	10531352	A nine-residue aspartate-containing peptide was obtained from the metalloproteinase that, when cyclized through the addition of terminal cysteines and oxidized to form a disulfide bond, was found to inhibit collagen binding to the alpha2 I-domain.	bind
45701	5	11383	5	NULL	NULL	NULL	NULL	statement 4	AminoAcid		forms					disulfide bond					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_44_31493_s_36	10531352	A nine-residue aspartate-containing peptide was obtained from the metalloproteinase that, when cyclized through the addition of terminal cysteines and oxidized to form a disulfide bond, was found to inhibit collagen binding to the alpha2 I-domain.	bind
45702	6	11383	5	NULL	NULL	NULL	NULL	statement 5	Process		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_44_31493_s_36	10531352	A nine-residue aspartate-containing peptide was obtained from the metalloproteinase that, when cyclized through the addition of terminal cysteines and oxidized to form a disulfide bond, was found to inhibit collagen binding to the alpha2 I-domain.	bind
46061	1	11383	6	10	NULL	0	NULL	collagen			bind					alpha2			I-domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_44_31493_s_36	10531352	A nine-residue aspartate-containing peptide was obtained from the metalloproteinase that, when cyclized through the addition of terminal cysteines and oxidized to form a disulfide bond, was found to inhibit collagen binding to the alpha2 I-domain.	bind
46063	2	11383	6	NULL	NULL	0	NULL	aspartate-containing peptide	NULL		is derived from	NULL				metalloproteinase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_44_31493_s_36	10531352	A nine-residue aspartate-containing peptide was obtained from the metalloproteinase that, when cyclized through the addition of terminal cysteines and oxidized to form a disulfide bond, was found to inhibit collagen binding to the alpha2 I-domain.	bind
46064	6	11383	6	10	NULL	0	NULL	statement 5	NULL		inhibits	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_44_31493_s_36	10531352	A nine-residue aspartate-containing peptide was obtained from the metalloproteinase that, when cyclized through the addition of terminal cysteines and oxidized to form a disulfide bond, was found to inhibit collagen binding to the alpha2 I-domain.	bind
51509	3	11383	6	10	NULL	0	NULL	statement 2	NULL		is cyclized through	NULL				cysteines	NULL	addition of ;;terminal			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_44_31493_s_36	10531352	A nine-residue aspartate-containing peptide was obtained from the metalloproteinase that, when cyclized through the addition of terminal cysteines and oxidized to form a disulfide bond, was found to inhibit collagen binding to the alpha2 I-domain.	bind
51511	4	11383	6	10	NULL	0	NULL	statement 3	NULL		undergoes	NULL				oxidation	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_44_31493_s_36	10531352	A nine-residue aspartate-containing peptide was obtained from the metalloproteinase that, when cyclized through the addition of terminal cysteines and oxidized to form a disulfide bond, was found to inhibit collagen binding to the alpha2 I-domain.	bind
51512	5	11383	6	10	NULL	0	NULL	statement 4	NULL		forms	NULL				disulfide bond	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_44_31493_s_36	10531352	A nine-residue aspartate-containing peptide was obtained from the metalloproteinase that, when cyclized through the addition of terminal cysteines and oxidized to form a disulfide bond, was found to inhibit collagen binding to the alpha2 I-domain.	bind
45703	1	11384	5	NULL	NULL	NULL	NULL	LDL	GP	acetylated	bind					pBR322 plasmid DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_drug-deliv_10_3_12944143_s_6	12944143	A nitrocellulose  filter-binding assay revealed that acetylated LDL bound approximately  25% of the [3]-labeled pBR322 plasmid DNA bound by native LDL under the  same conditions.	bind
45704	2	11384	5	NULL	NULL	NULL	NULL	LDL	GP	native	bind					pBR322 plasmid DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_drug-deliv_10_3_12944143_s_6	12944143	A nitrocellulose  filter-binding assay revealed that acetylated LDL bound approximately  25% of the [3]-labeled pBR322 plasmid DNA bound by native LDL under the  same conditions.	bind
46065	1	11384	6	NULL	NULL	0	NULL	LDL	NULL	acetylated	bind	NULL				pBR322 plasmid DNA	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_drug-deliv_10_3_12944143_s_6	12944143	A nitrocellulose  filter-binding assay revealed that acetylated LDL bound approximately  25% of the [3]-labeled pBR322 plasmid DNA bound by native LDL under the  same conditions.	bind
46066	2	11384	6	NULL	NULL	0	NULL	LDL	NULL	native	bind	NULL				pBR322 plasmid DNA	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_drug-deliv_10_3_12944143_s_6	12944143	A nitrocellulose  filter-binding assay revealed that acetylated LDL bound approximately  25% of the [3]-labeled pBR322 plasmid DNA bound by native LDL under the  same conditions.	bind
45705	1	11385	5	NULL	NULL	NULL	NULL	coat protein	GP		bind					21 nucleotide RNA fragment	NucleicAcid	synthetic			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-biomol-struct-dyn_1_2_6401118_s_3	6401118	A nitrocellulose filter retention assay is used  to demonstrate equimolar binding between the coat protein and a synthetic  21 nucleotide RNA fragment.	bind
46067	1	11385	6	10	NULL	0	NULL	coat protein	NULL		bind	NULL				21 nucleotide RNA fragment	NULL	synthetic 			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_j-biomol-struct-dyn_1_2_6401118_s_3	6401118	A nitrocellulose filter retention assay is used  to demonstrate equimolar binding between the coat protein and a synthetic  21 nucleotide RNA fragment.	bind
45706	1	11386	5	NULL	NULL	NULL	NULL	Chl	Chemical		bind					Chl aP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_50_32174_s_182	8943272	A nitrogen-containing amino acid side chain in His, Asn, or Gln may act as the 5th ligand during the binding of Chl or Zn-phe to the Chl  aP ( 35).	bind
45707	2	11386	5	NULL	NULL	NULL	NULL	Zn-phe	Chemical		bind					Chl aP	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_50_32174_s_182	8943272	A nitrogen-containing amino acid side chain in His, Asn, or Gln may act as the 5th ligand during the binding of Chl or Zn-phe to the Chl  aP ( 35).	bind
45708	3	11386	5	NULL	NULL	NULL	NULL	His	AminoAcid		acts as			nitrogen-containing amino acid side chain		statement 1	Process	ligand in			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_50_32174_s_182	8943272	A nitrogen-containing amino acid side chain in His, Asn, or Gln may act as the 5th ligand during the binding of Chl or Zn-phe to the Chl  aP ( 35).	bind
45709	4	11386	5	NULL	NULL	NULL	NULL	His	AminoAcid		acts as			amino acid side chains		statement 2	Process	ligand in			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_50_32174_s_182	8943272	A nitrogen-containing amino acid side chain in His, Asn, or Gln may act as the 5th ligand during the binding of Chl or Zn-phe to the Chl  aP ( 35).	bind
45710	5	11386	5	NULL	NULL	NULL	NULL	Asn	AminoAcid		acts as			nitrogen-containing amino acid side chain		statement 1	Process	ligand in			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_50_32174_s_182	8943272	A nitrogen-containing amino acid side chain in His, Asn, or Gln may act as the 5th ligand during the binding of Chl or Zn-phe to the Chl  aP ( 35).	bind
45711	6	11386	5	NULL	NULL	NULL	NULL	Asn	AminoAcid		acts as			nitrogen-containing amino acid side chain		statement 2	Process	ligand in			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_50_32174_s_182	8943272	A nitrogen-containing amino acid side chain in His, Asn, or Gln may act as the 5th ligand during the binding of Chl or Zn-phe to the Chl  aP ( 35).	bind
45712	7	11386	5	NULL	NULL	NULL	NULL	Gln	AminoAcid		acts as			nitrogen-containing amino acid side chain		statement 1	Process	ligand in			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_50_32174_s_182	8943272	A nitrogen-containing amino acid side chain in His, Asn, or Gln may act as the 5th ligand during the binding of Chl or Zn-phe to the Chl  aP ( 35).	bind
45713	8	11386	5	NULL	NULL	NULL	NULL	Gln	AminoAcid		acts as			nitrogen-containing amino acid side chain		statement 2	Process	ligand in			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_50_32174_s_182	8943272	A nitrogen-containing amino acid side chain in His, Asn, or Gln may act as the 5th ligand during the binding of Chl or Zn-phe to the Chl  aP ( 35).	bind
46068	1	11386	6	NULL	NULL	0	NULL	Chl	NULL		bind	NULL				Zn-phe	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_50_32174_s_182	8943272	A nitrogen-containing amino acid side chain in His, Asn, or Gln may act as the 5th ligand during the binding of Chl or Zn-phe to the Chl  aP ( 35).	bind
46069	2	11386	6	NULL	NULL	0	NULL	Chl	NULL		bind	NULL				Chl aP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_50_32174_s_182	8943272	A nitrogen-containing amino acid side chain in His, Asn, or Gln may act as the 5th ligand during the binding of Chl or Zn-phe to the Chl  aP ( 35).	bind
52939	3	11386	6	10	NULL	0	NULL	His	NULL		acts as a ligand in	NULL		nitrogen-containing amino acid side chain		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_50_32174_s_182	8943272	A nitrogen-containing amino acid side chain in His, Asn, or Gln may act as the 5th ligand during the binding of Chl or Zn-phe to the Chl  aP ( 35).	bind
52949	4	11386	6	NULL	NULL	0	NULL	His	NULL		acts as a ligand in	NULL		nitrogen-containing amino acid side chain		statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_50_32174_s_182	8943272	A nitrogen-containing amino acid side chain in His, Asn, or Gln may act as the 5th ligand during the binding of Chl or Zn-phe to the Chl  aP ( 35).	bind
52950	5	11386	6	NULL	NULL	0	NULL	Asn	NULL		acts as a ligand in	NULL		nitrogen-containing amino acid side chain		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_50_32174_s_182	8943272	A nitrogen-containing amino acid side chain in His, Asn, or Gln may act as the 5th ligand during the binding of Chl or Zn-phe to the Chl  aP ( 35).	bind
52951	6	11386	6	NULL	NULL	0	NULL	Asn	NULL		acts as a ligand in	NULL		nitrogen-containing amino acid side chain		statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_50_32174_s_182	8943272	A nitrogen-containing amino acid side chain in His, Asn, or Gln may act as the 5th ligand during the binding of Chl or Zn-phe to the Chl  aP ( 35).	bind
52952	7	11386	6	NULL	NULL	0	NULL	Gln	NULL		acts as a ligand in	NULL		nitrogen-containing amino acid side chain		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_50_32174_s_182	8943272	A nitrogen-containing amino acid side chain in His, Asn, or Gln may act as the 5th ligand during the binding of Chl or Zn-phe to the Chl  aP ( 35).	bind
52953	8	11386	6	NULL	NULL	0	NULL	Gln	NULL		acts as a ligand in	NULL		nitrogen-containing amino acid side chain		statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_50_32174_s_182	8943272	A nitrogen-containing amino acid side chain in His, Asn, or Gln may act as the 5th ligand during the binding of Chl or Zn-phe to the Chl  aP ( 35).	bind
45714	1	11387	5	NULL	NULL	NULL	NULL	nod factor	Chemical	legume roots	bind					lectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_64_1_180_s_883	10704479	A nod factor binding lectin with apyrase activity from legume roots.	bind
45715	2	11387	5	NULL	NULL	NULL	NULL	statement 1	Process	legume roots	demonstrate					apyrase activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_64_1_180_s_883	10704479	A nod factor binding lectin with apyrase activity from legume roots.	bind
46070	1	11387	6	NULL	NULL	0	NULL	nod factor	NULL	legume roots	bind	NULL				lectin	NULL				NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_64_1_180_s_883	10704479	A nod factor binding lectin with apyrase activity from legume roots.	bind
46071	2	11387	6	NULL	NULL	0	NULL	nod factor	NULL	legume roots	exhibits	NULL				apyrase activity	NULL				NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_64_1_180_s_883	10704479	A nod factor binding lectin with apyrase activity from legume roots.	bind
45716	1	11388	5	NULL	NULL	NULL	NULL	CNQX	Chemical		is an antagonist of					non- N-methyl-D-aspartate ionotropic glutamate receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_56_2_429_s_101	10419564	A non- N-methyl-D-aspartate ionotropic glutamate receptor antagonist, CNQX, also displaced [3]MGA (30 nM) binding, with a  Ki value of 1.4 muM ( n = 3).	bind
45717	2	11388	5	NULL	NULL	NULL	NULL	CNQX	Chemical		displaces					MGA	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_56_2_429_s_101	10419564	A non- N-methyl-D-aspartate ionotropic glutamate receptor antagonist, CNQX, also displaced [3]MGA (30 nM) binding, with a  Ki value of 1.4 muM ( n = 3).	bind
46072	1	11388	6	10	NULL	0	NULL	CNQX	NULL		is an antagonist of	NULL				non- N-methyl-D-aspartate ionotropic glutamate receptor antagonist	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_56_2_429_s_101	10419564	A non- N-methyl-D-aspartate ionotropic glutamate receptor antagonist, CNQX, also displaced [3]MGA (30 nM) binding, with a  Ki value of 1.4 muM ( n = 3).	bind
46073	2	11388	6	NULL	NULL	0	NULL	CNQX	NULL		displaces	NULL				MGA	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_56_2_429_s_101	10419564	A non- N-methyl-D-aspartate ionotropic glutamate receptor antagonist, CNQX, also displaced [3]MGA (30 nM) binding, with a  Ki value of 1.4 muM ( n = 3).	bind
45719	1	11389	5	NULL	NULL	NULL	NULL	receptor	GP	non-native disulfide bond;;mutant	destabilize			C35A		receptor	GP	Ang II binding state of			NULL		NULL	NULL	NULL	NULL	gw60_febslett_484_2_133_s_182	11068047	A non-native disulfide bond thus formed in both C35A and C290A mutant receptors could destabilize the Ang II binding state of the receptor.	bind
45720	2	11389	5	NULL	NULL	NULL	NULL	receptor	GP	non-native disulfide bond;;mutant	destabilize			C290A		receptor	GP	Ang II binding state of			NULL		NULL	NULL	NULL	NULL	gw60_febslett_484_2_133_s_182	11068047	A non-native disulfide bond thus formed in both C35A and C290A mutant receptors could destabilize the Ang II binding state of the receptor.	bind
46074	1	11389	6	10	NULL	0	NULL	receptor	NULL	non-native disulfide bond;;mutant	destabilize	NULL		C35A		receptor	NULL	Ang II binding state of 			NULL		NULL	NULL	NULL	NULL	gw60_febslett_484_2_133_s_182	11068047	A non-native disulfide bond thus formed in both C35A and C290A mutant receptors could destabilize the Ang II binding state of the receptor.	bind
46075	2	11389	6	10	NULL	0	NULL	receptor	NULL	non-native disulfide bond;;mutant	destabilize	NULL		 C290A		receptor	NULL	Ang II binding state of			NULL		NULL	NULL	NULL	NULL	gw60_febslett_484_2_133_s_182	11068047	A non-native disulfide bond thus formed in both C35A and C290A mutant receptors could destabilize the Ang II binding state of the receptor.	bind
45721	1	11390	5	NULL	NULL	NULL	NULL	hamartin	GP	non-phosphorylatable;;alanine substitution mutant	does not interact with			T310		Plk1	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_hum-mol-genet_15_2_16339216_s_8	16339216	A non-phosphorylatable hamartin  mutant with an alanine substitution at residue T310 does not interact  with Plk1, whereas a non-phosphorylatable hamartin mutant at residue S332  in conjunction with alanine mutations at the other CDC2/cyclin B1 sites  (T417, S584 and T1047) does not impact hamartin binding to Plk1.	bind
45722	2	11390	5	NULL	NULL	NULL	NULL	hamartin	GP		bind					Plk1	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_hum-mol-genet_15_2_16339216_s_8	16339216	A non-phosphorylatable hamartin  mutant with an alanine substitution at residue T310 does not interact  with Plk1, whereas a non-phosphorylatable hamartin mutant at residue S332  in conjunction with alanine mutations at the other CDC2/cyclin B1 sites  (T417, S584 and T1047) does not impact hamartin binding to Plk1.	bind
45723	3	11390	5	NULL	NULL	NULL	NULL	hamartin	GP	non-phosphorylatable;;mutant	undergoes			S332				alanine mutations at	CDC2/cyclin B1 sites		NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_hum-mol-genet_15_2_16339216_s_8	16339216	A non-phosphorylatable hamartin  mutant with an alanine substitution at residue T310 does not interact  with Plk1, whereas a non-phosphorylatable hamartin mutant at residue S332  in conjunction with alanine mutations at the other CDC2/cyclin B1 sites  (T417, S584 and T1047) does not impact hamartin binding to Plk1.	bind
45724	4	11390	5	10	NULL	0	NULL		NULL	alanine mutations	constitute	NULL		CDC2/cyclin B1 sites			NULL		T417;;S584;;T1047		NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_hum-mol-genet_15_2_16339216_s_8	16339216	A non-phosphorylatable hamartin  mutant with an alanine substitution at residue T310 does not interact  with Plk1, whereas a non-phosphorylatable hamartin mutant at residue S332  in conjunction with alanine mutations at the other CDC2/cyclin B1 sites  (T417, S584 and T1047) does not impact hamartin binding to Plk1.	bind
45725	5	11390	5	NULL	NULL	NULL	NULL	statement 3	Process		does not impact					statement 2	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_hum-mol-genet_15_2_16339216_s_8	16339216	A non-phosphorylatable hamartin  mutant with an alanine substitution at residue T310 does not interact  with Plk1, whereas a non-phosphorylatable hamartin mutant at residue S332  in conjunction with alanine mutations at the other CDC2/cyclin B1 sites  (T417, S584 and T1047) does not impact hamartin binding to Plk1.	bind
46131	1	11390	6	NULL	NULL	0	NULL	hamartin	NULL		is substituted by	NULL		alanine		hamartin	NULL		T310		NULL		0	NULL	NULL	NULL	abs-batch0600-0619_hum-mol-genet_15_2_16339216_s_8	16339216	A non-phosphorylatable hamartin  mutant with an alanine substitution at residue T310 does not interact  with Plk1, whereas a non-phosphorylatable hamartin mutant at residue S332  in conjunction with alanine mutations at the other CDC2/cyclin B1 sites  (T417, S584 and T1047) does not impact hamartin binding to Plk1.	bind
46132	2	11390	6	NULL	NULL	0	NULL	statement 1	NULL		does not bind	NULL				Plk1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0600-0619_hum-mol-genet_15_2_16339216_s_8	16339216	A non-phosphorylatable hamartin  mutant with an alanine substitution at residue T310 does not interact  with Plk1, whereas a non-phosphorylatable hamartin mutant at residue S332  in conjunction with alanine mutations at the other CDC2/cyclin B1 sites  (T417, S584 and T1047) does not impact hamartin binding to Plk1.	bind
46133	3	11390	6	NULL	NULL	0	NULL	hamartin	NULL		bind	NULL				Plk1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0600-0619_hum-mol-genet_15_2_16339216_s_8	16339216	A non-phosphorylatable hamartin  mutant with an alanine substitution at residue T310 does not interact  with Plk1, whereas a non-phosphorylatable hamartin mutant at residue S332  in conjunction with alanine mutations at the other CDC2/cyclin B1 sites  (T417, S584 and T1047) does not impact hamartin binding to Plk1.	bind
46134	4	11390	6	NULL	NULL	0	NULL	hamartin	NULL	mutant	acts in conjunction with	NULL		S332			NULL		T417;; S584;; T1047		NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_hum-mol-genet_15_2_16339216_s_8	16339216	A non-phosphorylatable hamartin  mutant with an alanine substitution at residue T310 does not interact  with Plk1, whereas a non-phosphorylatable hamartin mutant at residue S332  in conjunction with alanine mutations at the other CDC2/cyclin B1 sites  (T417, S584 and T1047) does not impact hamartin binding to Plk1.	bind
46135	5	11390	6	NULL	NULL	0	NULL	statement 4	NULL		does not impact	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	abs-batch0600-0619_hum-mol-genet_15_2_16339216_s_8	16339216	A non-phosphorylatable hamartin  mutant with an alanine substitution at residue T310 does not interact  with Plk1, whereas a non-phosphorylatable hamartin mutant at residue S332  in conjunction with alanine mutations at the other CDC2/cyclin B1 sites  (T417, S584 and T1047) does not impact hamartin binding to Plk1.	bind
60572	1	11393	5	NULL	NULL	NULL	NULL	ss genomes \t	NucleicAcid		does not bind					protein A	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_12_3282_s_125	11406604	A non-specific binding of ss genomes or capsids to the protein A - Sepharose was, however, not detected (data not shown).	bind
60573	2	11393	5	NULL	NULL	NULL	NULL	capsids	GP		does not bind					protein A	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_12_3282_s_125	11406604	A non-specific binding of ss genomes or capsids to the protein A - Sepharose was, however, not detected (data not shown).	bind
46077	1	11393	6	NULL	NULL	0	NULL	ss genomes	NULL		does not bind	NULL				protein A	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_20_12_3282_s_125	11406604	A non-specific binding of ss genomes or capsids to the protein A - Sepharose was, however, not detected (data not shown).	bind
46078	2	11393	6	NULL	NULL	0	NULL	capsids	NULL		does not bind	NULL				protein A	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_20_12_3282_s_125	11406604	A non-specific binding of ss genomes or capsids to the protein A - Sepharose was, however, not detected (data not shown).	bind
45728	1	11394	5	NULL	NULL	NULL	NULL	F3	AminoAcid		bind					TR2	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_310_2_384_s_99	14521922	A non-specific protein (BSA,  1  g) failed to affect the binding of F3 to TR2 (data not shown).	bind
45729	2	11394	5	NULL	NULL	NULL	NULL	BSA	GP		does not affect					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_310_2_384_s_99	14521922	A non-specific protein (BSA,  1  g) failed to affect the binding of F3 to TR2 (data not shown).	bind
45730	3	11394	5	NULL	NULL	NULL	NULL	BSA	GP		is a type of					non-specific protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_310_2_384_s_99	14521922	A non-specific protein (BSA,  1  g) failed to affect the binding of F3 to TR2 (data not shown).	bind
46079	1	11394	6	NULL	NULL	0	NULL	F3	NULL		bind	NULL				TR2	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_310_2_384_s_99	14521922	A non-specific protein (BSA,  1  g) failed to affect the binding of F3 to TR2 (data not shown).	bind
46080	2	11394	6	10	NULL	0	NULL	BSA	NULL		does not affect	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_310_2_384_s_99	14521922	A non-specific protein (BSA,  1  g) failed to affect the binding of F3 to TR2 (data not shown).	bind
51513	3	11394	6	10	NULL	0	NULL	BSA	NULL		is a type of	NULL				non-specific protein	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_310_2_384_s_99	14521922	A non-specific protein (BSA,  1  g) failed to affect the binding of F3 to TR2 (data not shown).	bind
45731	1	11396	5	NULL	NULL	NULL	NULL	 LOS structures	Chemical	gonococcal	bind					Opa proteins	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_infect-immun_63_4_7890406_s_3	7890406	A noncompetitive inhibition assay used previously to determine  the carbohydrate structures recognized by the major hepatic asialoglycoprotein  receptor was modified to determine the gonococcal LOS structures that  bind Opa proteins (R. T. Lee, Targeted Diagn.	bind
46081	1	11396	6	NULL	NULL	0	NULL	LOS structures	NULL	gonococcal	bind	NULL				Opa proteins	NULL				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_infect-immun_63_4_7890406_s_3	7890406	A noncompetitive inhibition assay used previously to determine  the carbohydrate structures recognized by the major hepatic asialoglycoprotein  receptor was modified to determine the gonococcal LOS structures that  bind Opa proteins (R. T. Lee, Targeted Diagn.	bind
45732	1	11397	5	NULL	NULL	NULL	NULL	TSH	GP		bind		high affinity			TSHR	GP				NULL	293 human embryonal kidney cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33423_s_164	9837919	A nonessential role of galactose and sialic acid in function of TSHR shown in Lec8 cells is reminiscent of our previous finding ( 4,  40) of high affinity TSH binding to TSHR expressed in 293 human embryonal kidney cells.	bind
46082	1	11397	6	NULL	NULL	0	NULL	TSH	NULL		bind	NULL	high affinity			TSHR	NULL				NULL	293 human embryonal kidney cells	0	NULL	NULL	NULL	gw60_jbiolchem_273_50_33423_s_164	9837919	A nonessential role of galactose and sialic acid in function of TSHR shown in Lec8 cells is reminiscent of our previous finding ( 4,  40) of high affinity TSH binding to TSHR expressed in 293 human embryonal kidney cells.	bind
45733	1	11398	5	NULL	NULL	NULL	NULL	68-kDa alpha-L-fucosidase	GP	nonglycosylated	bind					sperm	Cell	Unio elongatulus;;plasma membrane of			NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_68_3_709_s_281	12604617	A nonglycosylated, 68-kDa alpha-L-fucosidase is bound to the mollusc bivalve  Unio elongatulus sperm plasma membrane and differs from a glycosylated 56-kDa form present in the seminal fluid.	bind
45734	2	11398	5	NULL	NULL	NULL	NULL	Unio elongatulus	Organism		is a type of	Organism				mollusc bivalve	Organism				NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_68_3_709_s_281	12604617	A nonglycosylated, 68-kDa alpha-L-fucosidase is bound to the mollusc bivalve  Unio elongatulus sperm plasma membrane and differs from a glycosylated 56-kDa form present in the seminal fluid.	bind
45735	3	11398	5	NULL	NULL	NULL	NULL	56-kDa alpha-L-fucosidase		glycosylated	is present in					seminal fluid	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_68_3_709_s_281	12604617	A nonglycosylated, 68-kDa alpha-L-fucosidase is bound to the mollusc bivalve  Unio elongatulus sperm plasma membrane and differs from a glycosylated 56-kDa form present in the seminal fluid.	bind
45736	4	11398	5	NULL	NULL	NULL	NULL	statement 1	Process		differs from					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_68_3_709_s_281	12604617	A nonglycosylated, 68-kDa alpha-L-fucosidase is bound to the mollusc bivalve  Unio elongatulus sperm plasma membrane and differs from a glycosylated 56-kDa form present in the seminal fluid.	bind
46083	1	11398	6	NULL	NULL	0	NULL	alpha-L-fucosidase	NULL	nonglycoylated	bind	NULL				sperm plasma membrane	NULL	Unio elongatulus			NULL		0	NULL	NULL	NULL	gw60_biolreprod_68_3_709_s_281	12604617	A nonglycosylated, 68-kDa alpha-L-fucosidase is bound to the mollusc bivalve  Unio elongatulus sperm plasma membrane and differs from a glycosylated 56-kDa form present in the seminal fluid.	bind
46084	2	11398	6	10	NULL	0	NULL	Unio elongatulus	NULL		is a type of	NULL				mollusc bivalve	NULL				NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_68_3_709_s_281	12604617	A nonglycosylated, 68-kDa alpha-L-fucosidase is bound to the mollusc bivalve  Unio elongatulus sperm plasma membrane and differs from a glycosylated 56-kDa form present in the seminal fluid.	bind
51514	3	11398	6	10	NULL	0	NULL	56-kDa alpha-L-fucosidase	NULL	glycosylated	is present in	NULL				seminal fluid	NULL				NULL		0	NULL	NULL	NULL	gw60_biolreprod_68_3_709_s_281	12604617	A nonglycosylated, 68-kDa alpha-L-fucosidase is bound to the mollusc bivalve  Unio elongatulus sperm plasma membrane and differs from a glycosylated 56-kDa form present in the seminal fluid.	bind
45737	1	11399	5	NULL	NULL	NULL	NULL	OFQ-R	GP		bind					G proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_51_5_816_s_10	9145920	A nonhydrolyzable GTP analog [guanosine-5 -(beta,gamma-imido)triphosphate] reduced the affinity of both OFQ ligands to their receptor without significant changes in the total binding capacity, indicating functional interactions between the OFQ-R and G proteins.	bind
45738	2	11399	5	NULL	NULL	NULL	NULL	OFQ ligands	GP		bind					receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_51_5_816_s_10	9145920	A nonhydrolyzable GTP analog [guanosine-5 -(beta,gamma-imido)triphosphate] reduced the affinity of both OFQ ligands to their receptor without significant changes in the total binding capacity, indicating functional interactions between the OFQ-R and G proteins.	bind
45739	3	11399	5	NULL	NULL	NULL	NULL	guanosine-5 -(beta,gamma-imido)triphosphate	Chemical		is an analog of					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_51_5_816_s_10	9145920	A nonhydrolyzable GTP analog [guanosine-5 -(beta,gamma-imido)triphosphate] reduced the affinity of both OFQ ligands to their receptor without significant changes in the total binding capacity, indicating functional interactions between the OFQ-R and G proteins.	bind
45740	4	11399	5	NULL	NULL	NULL	NULL	statement 3	Chemical		reduce					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_51_5_816_s_10	9145920	A nonhydrolyzable GTP analog [guanosine-5 -(beta,gamma-imido)triphosphate] reduced the affinity of both OFQ ligands to their receptor without significant changes in the total binding capacity, indicating functional interactions between the OFQ-R and G proteins.	bind
46085	1	11399	6	NULL	NULL	0	NULL	OFQ-R 	NULL		bind	NULL				G protein	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_51_5_816_s_10	9145920	A nonhydrolyzable GTP analog [guanosine-5 -(beta,gamma-imido)triphosphate] reduced the affinity of both OFQ ligands to their receptor without significant changes in the total binding capacity, indicating functional interactions between the OFQ-R and G proteins.	bind
46086	2	11399	6	10	NULL	0	NULL	guanosine-5 -(beta,gamma-imido)triphosphate	NULL		is a type of	NULL				GTP analog	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_51_5_816_s_10	9145920	A nonhydrolyzable GTP analog [guanosine-5 -(beta,gamma-imido)triphosphate] reduced the affinity of both OFQ ligands to their receptor without significant changes in the total binding capacity, indicating functional interactions between the OFQ-R and G proteins.	bind
46087	4	11399	6	10	NULL	0	NULL	statement 2	NULL		reduces	NULL				statement 3	NULL	affinity of			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_51_5_816_s_10	9145920	A nonhydrolyzable GTP analog [guanosine-5 -(beta,gamma-imido)triphosphate] reduced the affinity of both OFQ ligands to their receptor without significant changes in the total binding capacity, indicating functional interactions between the OFQ-R and G proteins.	bind
51515	3	11399	6	10	NULL	0	NULL	OFQ ligands	NULL		bind	NULL				receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_51_5_816_s_10	9145920	A nonhydrolyzable GTP analog [guanosine-5 -(beta,gamma-imido)triphosphate] reduced the affinity of both OFQ ligands to their receptor without significant changes in the total binding capacity, indicating functional interactions between the OFQ-R and G proteins.	bind
45741	1	11400	5	NULL	NULL	NULL	NULL	Fl-APC	GP		bind					E-7 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_29_17491_s_176	8663475	A noninhibitory antibody (HPC2) was used to immobilize protein C. HPC2 is a calcium-independent, anti-human protein C IgG1 monoclonal antibody that also reacts with human APC. HPC2 does not inhibit Fl-APC binding to E-7 cells.	bind
45742	2	11400	5	NULL	NULL	NULL	NULL	HPC2	GP		does not inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_29_17491_s_176	8663475	A noninhibitory antibody (HPC2) was used to immobilize protein C. HPC2 is a calcium-independent, anti-human protein C IgG1 monoclonal antibody that also reacts with human APC. HPC2 does not inhibit Fl-APC binding to E-7 cells.	bind
45743	3	11400	5	NULL	NULL	NULL	NULL	HPC2	GP		is a type of					noninhibitory antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_29_17491_s_176	8663475	A noninhibitory antibody (HPC2) was used to immobilize protein C. HPC2 is a calcium-independent, anti-human protein C IgG1 monoclonal antibody that also reacts with human APC. HPC2 does not inhibit Fl-APC binding to E-7 cells.	bind
45744	4	11400	5	NULL	NULL	NULL	NULL	HPC2	GP		is a type of					anti-human protein C IgG1 monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_29_17491_s_176	8663475	A noninhibitory antibody (HPC2) was used to immobilize protein C. HPC2 is a calcium-independent, anti-human protein C IgG1 monoclonal antibody that also reacts with human APC. HPC2 does not inhibit Fl-APC binding to E-7 cells.	bind
45746	5	11400	5	NULL	NULL	NULL	NULL	HPC2	GP		is independent of					calcium	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_29_17491_s_176	8663475	A noninhibitory antibody (HPC2) was used to immobilize protein C. HPC2 is a calcium-independent, anti-human protein C IgG1 monoclonal antibody that also reacts with human APC. HPC2 does not inhibit Fl-APC binding to E-7 cells.	bind
45747	6	11400	5	NULL	NULL	NULL	NULL	HPC2	GP		reacts with					APC	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_29_17491_s_176	8663475	A noninhibitory antibody (HPC2) was used to immobilize protein C. HPC2 is a calcium-independent, anti-human protein C IgG1 monoclonal antibody that also reacts with human APC. HPC2 does not inhibit Fl-APC binding to E-7 cells.	bind
54087	7	11400	5	NULL	NULL	NULL	NULL	HPC2	GP		immobilize					protein C	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_29_17491_s_176	8663475	A noninhibitory antibody (HPC2) was used to immobilize protein C. HPC2 is a calcium-independent, anti-human protein C IgG1 monoclonal antibody that also reacts with human APC. HPC2 does not inhibit Fl-APC binding to E-7 cells.	bind
46088	1	11400	6	NULL	NULL	0	NULL	Fl-APC	NULL		bind	NULL				E-7 cells	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_29_17491_s_176	8663475	A noninhibitory antibody (HPC2) was used to immobilize protein C. HPC2 is a calcium-independent, anti-human protein C IgG1 monoclonal antibody that also reacts with human APC. HPC2 does not inhibit Fl-APC binding to E-7 cells.	bind
46089	2	11400	6	NULL	NULL	0	NULL	HPC2	NULL		does not inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_29_17491_s_176	8663475	A noninhibitory antibody (HPC2) was used to immobilize protein C. HPC2 is a calcium-independent, anti-human protein C IgG1 monoclonal antibody that also reacts with human APC. HPC2 does not inhibit Fl-APC binding to E-7 cells.	bind
46090	3	11400	6	NULL	NULL	0	NULL	HPC2	NULL		immobilize	NULL				protein C	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_29_17491_s_176	8663475	A noninhibitory antibody (HPC2) was used to immobilize protein C. HPC2 is a calcium-independent, anti-human protein C IgG1 monoclonal antibody that also reacts with human APC. HPC2 does not inhibit Fl-APC binding to E-7 cells.	bind
46091	4	11400	6	NULL	NULL	0	NULL	HPC2	NULL		is a type of	NULL				anti-human protein C IgG1 monoclonal antibody	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_29_17491_s_176	8663475	A noninhibitory antibody (HPC2) was used to immobilize protein C. HPC2 is a calcium-independent, anti-human protein C IgG1 monoclonal antibody that also reacts with human APC. HPC2 does not inhibit Fl-APC binding to E-7 cells.	bind
46092	5	11400	6	NULL	NULL	0	NULL	HPC2	NULL		is independent of	NULL				calcium	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_29_17491_s_176	8663475	A noninhibitory antibody (HPC2) was used to immobilize protein C. HPC2 is a calcium-independent, anti-human protein C IgG1 monoclonal antibody that also reacts with human APC. HPC2 does not inhibit Fl-APC binding to E-7 cells.	bind
51516	6	11400	6	10	NULL	0	NULL	HPC2	NULL		reacts with	NULL				APC	NULL	human			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_29_17491_s_176	8663475	A noninhibitory antibody (HPC2) was used to immobilize protein C. HPC2 is a calcium-independent, anti-human protein C IgG1 monoclonal antibody that also reacts with human APC. HPC2 does not inhibit Fl-APC binding to E-7 cells.	bind
51517	7	11400	6	10	NULL	0	NULL	HPC2	NULL		is a type of	NULL				noninhibitory antibody	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_29_17491_s_176	8663475	A noninhibitory antibody (HPC2) was used to immobilize protein C. HPC2 is a calcium-independent, anti-human protein C IgG1 monoclonal antibody that also reacts with human APC. HPC2 does not inhibit Fl-APC binding to E-7 cells.	bind
50823	1	11401	5	NULL	NULL	NULL	NULL	Nct1	NucleicAcid		is a type of					Nonprotein-Coding RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_73_4_840_s_119	15987823	A Nonprotein-Coding RNA (Nct1) Binds TSN	bind
50824	2	11401	5	NULL	NULL	NULL	NULL	Nct1	NucleicAcid		bind					TSN	GP				NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_73_4_840_s_119	15987823	A Nonprotein-Coding RNA (Nct1) Binds TSN	bind
47384	1	11401	6	NULL	NULL	0	NULL	Nct1	NULL		bind	NULL				TSN	NULL				NULL		0	NULL	NULL	NULL	gw70_biolreprod_73_4_840_s_119	15987823	A Nonprotein-Coding RNA (Nct1) Binds TSN	bind
47385	2	11401	6	10	NULL	0	NULL	Nct1			is a type of					Nonprotein-Coding RNA					NULL		NULL	NULL	NULL	NULL	gw70_biolreprod_73_4_840_s_119	15987823	A Nonprotein-Coding RNA (Nct1) Binds TSN	bind
50825	1	11403	5	NULL	NULL	NULL	NULL	Hm	Chemical		bind		high-affinity			P. gingivalis cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_8_2528_s_291	12670977	A notable exception is the blocking of high-affinity Hm binding to  P. gingivalis cells by competition with PPIX ( ), indicating that in this case an alternative to the general mechanism is operative and a significant fraction of heme acquisition must be mediated by a process which can capture nonmetal porphyrins.	bind
50826	2	11403	5	NULL	NULL	NULL	NULL	PPIX	Chemical		bind					P. gingivalis cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_8_2528_s_291	12670977	A notable exception is the blocking of high-affinity Hm binding to  P. gingivalis cells by competition with PPIX ( ), indicating that in this case an alternative to the general mechanism is operative and a significant fraction of heme acquisition must be mediated by a process which can capture nonmetal porphyrins.	bind
50827	3	11403	5	NULL	NULL	NULL	NULL	statement 1	Process		competes with					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_8_2528_s_291	12670977	A notable exception is the blocking of high-affinity Hm binding to  P. gingivalis cells by competition with PPIX ( ), indicating that in this case an alternative to the general mechanism is operative and a significant fraction of heme acquisition must be mediated by a process which can capture nonmetal porphyrins.	bind
50828	4	11403	5	NULL	NULL	NULL	NULL	statement 2	Process		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_8_2528_s_291	12670977	A notable exception is the blocking of high-affinity Hm binding to  P. gingivalis cells by competition with PPIX ( ), indicating that in this case an alternative to the general mechanism is operative and a significant fraction of heme acquisition must be mediated by a process which can capture nonmetal porphyrins.	bind
47393	1	11403	6	10	NULL	0	NULL	Hm			bind		high-affinity			P. gingivalis cells					NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_8_2528_s_291	12670977	A notable exception is the blocking of high-affinity Hm binding to  P. gingivalis cells by competition with PPIX ( ), indicating that in this case an alternative to the general mechanism is operative and a significant fraction of heme acquisition must be mediated by a process which can capture nonmetal porphyrins.	bind
47394	2	11403	6	NULL	NULL	0	NULL	PPIX	NULL		bind	NULL				P. gingivalis cells	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_8_2528_s_291	12670977	A notable exception is the blocking of high-affinity Hm binding to  P. gingivalis cells by competition with PPIX ( ), indicating that in this case an alternative to the general mechanism is operative and a significant fraction of heme acquisition must be mediated by a process which can capture nonmetal porphyrins.	bind
47395	3	11403	6	NULL	NULL	0	NULL	statement 1	NULL		competes	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_8_2528_s_291	12670977	A notable exception is the blocking of high-affinity Hm binding to  P. gingivalis cells by competition with PPIX ( ), indicating that in this case an alternative to the general mechanism is operative and a significant fraction of heme acquisition must be mediated by a process which can capture nonmetal porphyrins.	bind
54088	4	11403	6	10	NULL	0	NULL	statement 2			blocks					statement 1					NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_8_2528_s_291	12670977	A notable exception is the blocking of high-affinity Hm binding to  P. gingivalis cells by competition with PPIX ( ), indicating that in this case an alternative to the general mechanism is operative and a significant fraction of heme acquisition must be mediated by a process which can capture nonmetal porphyrins.	bind
50829	1	11405	5	NULL	NULL	NULL	NULL	Ag+	Chemical		acts as					SR Ca2+-releasing agent	Chemical	potent			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_11_7069_s_100	9054399	A notable exception is the effect of Ag+, which acts as a potent SR Ca2+-releasing agent at micromolar concentrations ( 4,  5), but decreases ryanodine binding by rapidly displacing bound ryanodine from its receptor ( 25).	bind
50830	2	11405	5	NULL	NULL	NULL	NULL	ryanodine	Chemical		bind					ryanodine receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_11_7069_s_100	9054399	A notable exception is the effect of Ag+, which acts as a potent SR Ca2+-releasing agent at micromolar concentrations ( 4,  5), but decreases ryanodine binding by rapidly displacing bound ryanodine from its receptor ( 25).	bind
50831	3	11405	5	NULL	NULL	NULL	NULL	ryanodine	Chemical		displaced from		rapidly			ryanodine receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_11_7069_s_100	9054399	A notable exception is the effect of Ag+, which acts as a potent SR Ca2+-releasing agent at micromolar concentrations ( 4,  5), but decreases ryanodine binding by rapidly displacing bound ryanodine from its receptor ( 25).	bind
50832	4	11405	5	NULL	NULL	NULL	NULL	Ag+	Chemical		decreases					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_11_7069_s_100	9054399	A notable exception is the effect of Ag+, which acts as a potent SR Ca2+-releasing agent at micromolar concentrations ( 4,  5), but decreases ryanodine binding by rapidly displacing bound ryanodine from its receptor ( 25).	bind
54091	5	11405	5	NULL	NULL	NULL	NULL	Ag+	Chemical		mediates					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_11_7069_s_100	9054399	A notable exception is the effect of Ag+, which acts as a potent SR Ca2+-releasing agent at micromolar concentrations ( 4,  5), but decreases ryanodine binding by rapidly displacing bound ryanodine from its receptor ( 25).	bind
47414	1	11405	6	NULL	NULL	0	NULL	Ag+	NULL		acts as a 	NULL				SR Ca2+-releasing agent	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_11_7069_s_100	9054399	A notable exception is the effect of Ag+, which acts as a potent SR Ca2+-releasing agent at micromolar concentrations ( 4,  5), but decreases ryanodine binding by rapidly displacing bound ryanodine from its receptor ( 25).	bind
47415	2	11405	6	NULL	NULL	0	NULL	ryanodine	NULL		bind	NULL				ryanodine receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_11_7069_s_100	9054399	A notable exception is the effect of Ag+, which acts as a potent SR Ca2+-releasing agent at micromolar concentrations ( 4,  5), but decreases ryanodine binding by rapidly displacing bound ryanodine from its receptor ( 25).	bind
47417	3	11405	6	NULL	NULL	0	NULL	Ag+	NULL		decreases	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_11_7069_s_100	9054399	A notable exception is the effect of Ag+, which acts as a potent SR Ca2+-releasing agent at micromolar concentrations ( 4,  5), but decreases ryanodine binding by rapidly displacing bound ryanodine from its receptor ( 25).	bind
54089	4	11405	6	10	NULL	0	NULL	ryanodine			displaced from		rapidly			ryanodine receptor					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_11_7069_s_100	9054399	A notable exception is the effect of Ag+, which acts as a potent SR Ca2+-releasing agent at micromolar concentrations ( 4,  5), but decreases ryanodine binding by rapidly displacing bound ryanodine from its receptor ( 25).	bind
54090	5	11405	6	10	NULL	0	NULL	Ag+			mediates					statement 4					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_11_7069_s_100	9054399	A notable exception is the effect of Ag+, which acts as a potent SR Ca2+-releasing agent at micromolar concentrations ( 4,  5), but decreases ryanodine binding by rapidly displacing bound ryanodine from its receptor ( 25).	bind
50833	1	11406	5	NULL	NULL	NULL	NULL	vitronectin	GP		bind					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1545_1_289_s_4	11342054	A notable interaction is the binding of vitronectin to heparin, inhibiting its characteristic rate enhancement on the thrombin/antithrombin reaction [  1.	bind
50834	2	11406	5	NULL	NULL	NULL	NULL	thrombin	GP		bind					antithrombin	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1545_1_289_s_4	11342054	A notable interaction is the binding of vitronectin to heparin, inhibiting its characteristic rate enhancement on the thrombin/antithrombin reaction [  1.	bind
47419	1	11406	6	NULL	NULL	0	NULL	vitronectin	NULL		bind	NULL				heparin	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1545_1_289_s_4	11342054	A notable interaction is the binding of vitronectin to heparin, inhibiting its characteristic rate enhancement on the thrombin/antithrombin reaction [  1.	bind
47422	2	11406	6	NULL	NULL	0	NULL	thrombin	NULL		bind	NULL				antithrombin	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1545_1_289_s_4	11342054	A notable interaction is the binding of vitronectin to heparin, inhibiting its characteristic rate enhancement on the thrombin/antithrombin reaction [  1.	bind
50835	1	11407	5	NULL	NULL	NULL	NULL	u-PA 	GP		bind					VLDL-R	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20855_s_241	7657671	A noteworthy  difference was observed with monoclonal anti-PAI-1 antibody from  hybridoma clone 2, which markedly stimulated binding of u-PA PAI-1  to VLDL-R but inhibited its binding alpha MR/LRP  alpha-chain.	bind
50836	2	11407	5	NULL	NULL	NULL	NULL	u-PA	GP		bind					alpha MR/LRP	GP		alpha-chain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20855_s_241	7657671	A noteworthy  difference was observed with monoclonal anti-PAI-1 antibody from  hybridoma clone 2, which markedly stimulated binding of u-PA PAI-1  to VLDL-R but inhibited its binding alpha MR/LRP  alpha-chain.	bind
50837	3	11407	5	NULL	NULL	NULL	NULL	monoclonal anti-PAI-1 antibody	GP		stimulates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20855_s_241	7657671	A noteworthy  difference was observed with monoclonal anti-PAI-1 antibody from  hybridoma clone 2, which markedly stimulated binding of u-PA PAI-1  to VLDL-R but inhibited its binding alpha MR/LRP  alpha-chain.	bind
50838	4	11407	5	NULL	NULL	NULL	NULL	monoclonal anti-PAI-1 antibody	GP		inhibit					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20855_s_241	7657671	A noteworthy  difference was observed with monoclonal anti-PAI-1 antibody from  hybridoma clone 2, which markedly stimulated binding of u-PA PAI-1  to VLDL-R but inhibited its binding alpha MR/LRP  alpha-chain.	bind
54092	5	11407	5	NULL	NULL	NULL	NULL	PAI-1	GP		bind					VLDL-R	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20855_s_241	7657671	A noteworthy  difference was observed with monoclonal anti-PAI-1 antibody from  hybridoma clone 2, which markedly stimulated binding of u-PA PAI-1  to VLDL-R but inhibited its binding alpha MR/LRP  alpha-chain.	bind
54093	6	11407	5	NULL	NULL	NULL	NULL	PAI-1	GP		bind					alpha MR/LRP	GP		alpha-chain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20855_s_241	7657671	A noteworthy  difference was observed with monoclonal anti-PAI-1 antibody from  hybridoma clone 2, which markedly stimulated binding of u-PA PAI-1  to VLDL-R but inhibited its binding alpha MR/LRP  alpha-chain.	bind
54094	7	11407	5	NULL	NULL	NULL	NULL	monoclonal anti-PAI-1 antibody	GP		stimulate					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20855_s_241	7657671	A noteworthy  difference was observed with monoclonal anti-PAI-1 antibody from  hybridoma clone 2, which markedly stimulated binding of u-PA PAI-1  to VLDL-R but inhibited its binding alpha MR/LRP  alpha-chain.	bind
54095	8	11407	5	NULL	NULL	NULL	NULL	monoclonal anti-PAI-1 antibody	GP		inhibit					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20855_s_241	7657671	A noteworthy  difference was observed with monoclonal anti-PAI-1 antibody from  hybridoma clone 2, which markedly stimulated binding of u-PA PAI-1  to VLDL-R but inhibited its binding alpha MR/LRP  alpha-chain.	bind
47805	1	11407	6	NULL	NULL	0	NULL	u-PA	NULL		bind	NULL				VLDL-R	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20855_s_241	7657671	A noteworthy  difference was observed with monoclonal anti-PAI-1 antibody from  hybridoma clone 2, which markedly stimulated binding of u-PA PAI-1  to VLDL-R but inhibited its binding alpha MR/LRP  alpha-chain.	bind
47806	2	11407	6	NULL	NULL	0	NULL	PAI-1	NULL		bind	NULL				VLDL-R	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20855_s_241	7657671	A noteworthy  difference was observed with monoclonal anti-PAI-1 antibody from  hybridoma clone 2, which markedly stimulated binding of u-PA PAI-1  to VLDL-R but inhibited its binding alpha MR/LRP  alpha-chain.	bind
47807	3	11407	6	10	NULL	0	NULL	monoclonal anti-PAI-1 antibody			stimulates					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20855_s_241	7657671	A noteworthy  difference was observed with monoclonal anti-PAI-1 antibody from  hybridoma clone 2, which markedly stimulated binding of u-PA PAI-1  to VLDL-R but inhibited its binding alpha MR/LRP  alpha-chain.	bind
47808	4	11407	6	10	NULL	0	NULL	monoclonal anti-PAI-1 antibody			stimulates					statement 2					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20855_s_241	7657671	A noteworthy  difference was observed with monoclonal anti-PAI-1 antibody from  hybridoma clone 2, which markedly stimulated binding of u-PA PAI-1  to VLDL-R but inhibited its binding alpha MR/LRP  alpha-chain.	bind
47809	5	11407	6	NULL	NULL	0	NULL	u-PA	NULL		bind	NULL				MR/LRP	NULL		alpha chain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20855_s_241	7657671	A noteworthy  difference was observed with monoclonal anti-PAI-1 antibody from  hybridoma clone 2, which markedly stimulated binding of u-PA PAI-1  to VLDL-R but inhibited its binding alpha MR/LRP  alpha-chain.	bind
47810	6	11407	6	NULL	NULL	0	NULL	PAI-1	NULL		bind	NULL				MR/LRP	NULL		alpha chain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20855_s_241	7657671	A noteworthy  difference was observed with monoclonal anti-PAI-1 antibody from  hybridoma clone 2, which markedly stimulated binding of u-PA PAI-1  to VLDL-R but inhibited its binding alpha MR/LRP  alpha-chain.	bind
47811	7	11407	6	10	NULL	0	NULL	monoclonal anti-PAI-1 antibody			inhibits					statement 5					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20855_s_241	7657671	A noteworthy  difference was observed with monoclonal anti-PAI-1 antibody from  hybridoma clone 2, which markedly stimulated binding of u-PA PAI-1  to VLDL-R but inhibited its binding alpha MR/LRP  alpha-chain.	bind
47812	8	11407	6	10	NULL	0	NULL	monoclonal anti-PAI-1 antibody			inhibits					statement 6					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20855_s_241	7657671	A noteworthy  difference was observed with monoclonal anti-PAI-1 antibody from  hybridoma clone 2, which markedly stimulated binding of u-PA PAI-1  to VLDL-R but inhibited its binding alpha MR/LRP  alpha-chain.	bind
50839	1	11409	5	NULL	NULL	NULL	NULL	96-kDa aminopeptidase	GP		is localized on					epithelial cell membranes	CellComponent	Bombyx mori;;midgut			NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_j-biochem-(tokyo)_139_2_16452310_s_1	16452310	A Novel 96-kDa Aminopeptidase Localized on Epithelial Cell Membranes of Bombyx mori Midgut, Which Binds to Cry1Ac Toxin of Bacillus thuringiensis..	bind
50840	2	11409	5	NULL	NULL	NULL	NULL	96-kDa aminopeptidase	GP		bind					Cry1Ac toxin	GP	Bacillus thuringiensis			NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_j-biochem-(tokyo)_139_2_16452310_s_1	16452310	A Novel 96-kDa Aminopeptidase Localized on Epithelial Cell Membranes of Bombyx mori Midgut, Which Binds to Cry1Ac Toxin of Bacillus thuringiensis..	bind
47474	1	11409	6	NULL	NULL	0	NULL	96-kDa Aminopeptidase	NULL		is localized on	NULL				Epithelial Cell Membranes	NULL	Bombyx mori;; Midgut			NULL		0	NULL	NULL	NULL	abs-batch0600-0619_j-biochem-(tokyo)_139_2_16452310_s_1	16452310	A Novel 96-kDa Aminopeptidase Localized on Epithelial Cell Membranes of Bombyx mori Midgut, Which Binds to Cry1Ac Toxin of Bacillus thuringiensis..	bind
47475	2	11409	6	NULL	NULL	0	NULL	96-kDa Aminopeptidase	NULL		bind	NULL				Cry1Ac Toxin	NULL	Bacillus thuringiensis			NULL		0	NULL	NULL	NULL	abs-batch0600-0619_j-biochem-(tokyo)_139_2_16452310_s_1	16452310	A Novel 96-kDa Aminopeptidase Localized on Epithelial Cell Membranes of Bombyx mori Midgut, Which Binds to Cry1Ac Toxin of Bacillus thuringiensis..	bind
50841	1	11410	5	NULL	NULL	NULL	NULL	Anti-beta 1 Integrin	GP		is a type of					Monoclonal Antibody	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_43_25570_s_316	7592728	A Novel Activating Anti-beta 1 Integrin Monoclonal Antibody Binds to the Cysteine-rich Repeats in the beta 1 Chain.	bind
50842	2	11410	5	NULL	NULL	NULL	NULL	Anti-beta 1 Integrin	GP		bind								Cysteine-rich Repeats in beta 1 Chain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_43_25570_s_316	7592728	A Novel Activating Anti-beta 1 Integrin Monoclonal Antibody Binds to the Cysteine-rich Repeats in the beta 1 Chain.	bind
47476	1	11410	6	NULL	NULL	0	NULL	Anti-beta 1 Integrin	NULL		is a type of	NULL				monoclonal antibody	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_43_25570_s_316	7592728	A Novel Activating Anti-beta 1 Integrin Monoclonal Antibody Binds to the Cysteine-rich Repeats in the beta 1 Chain.	bind
47477	2	11410	6	NULL	NULL	0	NULL	Anti-beta 1 Integrin	NULL		bind	NULL					NULL		Cysteine-rich Repeats in the beta 1 Chain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_43_25570_s_316	7592728	A Novel Activating Anti-beta 1 Integrin Monoclonal Antibody Binds to the Cysteine-rich Repeats in the beta 1 Chain.	bind
50843	1	11411	5	NULL	NULL	NULL	NULL	Kinase adapter 1	GP	Caenorhabditis elegans	bind		avidly			Protein kinase C3	GP				NULL		NULL	NULL	NULL	NULL	gw60_annrevneur_21_0_279_s_427	9530498	A Novel Adapter Protein Employs a Phosphotyrosine Binding Domain and Exceptionally Basic N-terminal Domains to Capture and Localize an Atypical Protein Kinase C. CHARACTERIZATION OF CAENORHABDITIS ELEGANS C KINASE ADAPTER 1, A PROTEIN THAT AVIDLY BINDS PROTEIN KINASE C3.	bind
50844	2	11411	5	NULL	NULL	NULL	NULL	Adapter protein	GP		employs								phosphotyrosine binding domain;;basic N-terminal domains		NULL		NULL	NULL	NULL	NULL	gw60_annrevneur_21_0_279_s_427	9530498	A Novel Adapter Protein Employs a Phosphotyrosine Binding Domain and Exceptionally Basic N-terminal Domains to Capture and Localize an Atypical Protein Kinase C. CHARACTERIZATION OF CAENORHABDITIS ELEGANS C KINASE ADAPTER 1, A PROTEIN THAT AVIDLY BINDS PROTEIN KINASE C3.	bind
50845	3	11411	5	NULL	NULL	NULL	NULL	statement 2	Process		is required for					protein kinase C 	GP	localization of			NULL		NULL	NULL	NULL	NULL	gw60_annrevneur_21_0_279_s_427	9530498	A Novel Adapter Protein Employs a Phosphotyrosine Binding Domain and Exceptionally Basic N-terminal Domains to Capture and Localize an Atypical Protein Kinase C. CHARACTERIZATION OF CAENORHABDITIS ELEGANS C KINASE ADAPTER 1, A PROTEIN THAT AVIDLY BINDS PROTEIN KINASE C3.	bind
47813	1	11411	6	NULL	NULL	0	NULL	Kinase Adaptor 1	NULL	Caenorhabditis elegans	bind	NULL	avidly			Protein kinase C3	NULL				NULL		0	NULL	NULL	NULL	gw60_annrevneur_21_0_279_s_427	9530498	A Novel Adapter Protein Employs a Phosphotyrosine Binding Domain and Exceptionally Basic N-terminal Domains to Capture and Localize an Atypical Protein Kinase C. CHARACTERIZATION OF CAENORHABDITIS ELEGANS C KINASE ADAPTER 1, A PROTEIN THAT AVIDLY BINDS PROTEIN KINASE C3.	bind
47814	2	11411	6	10	NULL	0	NULL	Adapter protein			employs								Phosphotyrosine Binding Domain;; Basic N-terminal Domain		NULL		NULL	NULL	NULL	NULL	gw60_annrevneur_21_0_279_s_427	9530498	A Novel Adapter Protein Employs a Phosphotyrosine Binding Domain and Exceptionally Basic N-terminal Domains to Capture and Localize an Atypical Protein Kinase C. CHARACTERIZATION OF CAENORHABDITIS ELEGANS C KINASE ADAPTER 1, A PROTEIN THAT AVIDLY BINDS PROTEIN KINASE C3.	bind
47815	3	11411	6	NULL	NULL	0	NULL	statement 2	NULL		is required for	NULL				protein kinase C	NULL	localization of 			NULL		0	NULL	NULL	NULL	gw60_annrevneur_21_0_279_s_427	9530498	A Novel Adapter Protein Employs a Phosphotyrosine Binding Domain and Exceptionally Basic N-terminal Domains to Capture and Localize an Atypical Protein Kinase C. CHARACTERIZATION OF CAENORHABDITIS ELEGANS C KINASE ADAPTER 1, A PROTEIN THAT AVIDLY BINDS PROTEIN KINASE C3.	bind
50846	1	11412	5	NULL	NULL	NULL	NULL	N2'' - Mad2	GP		bind					Mad1	GP				NULL	kinetochores	NULL	NULL	NULL	NULL	gw70_cellbiol_173_2_153_s_91	16636141	A novel and important extension of DeAntoni et al. (2005) was that the kinetochore localization of fluorescently labeled recombinant Mad2 injected into Ptk cells depends on its ability to dimerize with N2'' - Mad2 already bound to Mad1 at the kinetochores.	bind
50847	2	11412	5	NULL	NULL	NULL	NULL	Mad2	GP	recombinant	is localized in					kinetochore	CellComponent				NULL	Ptk cells	NULL	NULL	NULL	NULL	gw70_cellbiol_173_2_153_s_91	16636141	A novel and important extension of DeAntoni et al. (2005) was that the kinetochore localization of fluorescently labeled recombinant Mad2 injected into Ptk cells depends on its ability to dimerize with N2'' - Mad2 already bound to Mad1 at the kinetochores.	bind
50848	3	11412	5	NULL	NULL	NULL	NULL	Mad2	GP	recombinant	dimerize with					statement 1	Process				NULL	Ptk cells	NULL	NULL	NULL	NULL	gw70_cellbiol_173_2_153_s_91	16636141	A novel and important extension of DeAntoni et al. (2005) was that the kinetochore localization of fluorescently labeled recombinant Mad2 injected into Ptk cells depends on its ability to dimerize with N2'' - Mad2 already bound to Mad1 at the kinetochores.	bind
50849	4	11412	5	NULL	NULL	NULL	NULL	statement 2	Process		depends on					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_173_2_153_s_91	16636141	A novel and important extension of DeAntoni et al. (2005) was that the kinetochore localization of fluorescently labeled recombinant Mad2 injected into Ptk cells depends on its ability to dimerize with N2'' - Mad2 already bound to Mad1 at the kinetochores.	bind
47478	1	11412	6	NULL	NULL	0	NULL	N2'' - Mad2	NULL		bind	NULL				Mad1	NULL				NULL	kinetochores	0	NULL	NULL	NULL	gw70_cellbiol_173_2_153_s_91	16636141	A novel and important extension of DeAntoni et al. (2005) was that the kinetochore localization of fluorescently labeled recombinant Mad2 injected into Ptk cells depends on its ability to dimerize with N2'' - Mad2 already bound to Mad1 at the kinetochores.	bind
47479	2	11412	6	10	NULL	0	NULL	Mad2		recombinant	dimerizes with					statement 1					NULL	Ptk cells	NULL	NULL	NULL	NULL	gw70_cellbiol_173_2_153_s_91	16636141	A novel and important extension of DeAntoni et al. (2005) was that the kinetochore localization of fluorescently labeled recombinant Mad2 injected into Ptk cells depends on its ability to dimerize with N2'' - Mad2 already bound to Mad1 at the kinetochores.	bind
47480	3	11412	6	10	NULL	0	NULL	Mad2		recombinant	is localized on					kinetochore					NULL	Ptk cells	NULL	NULL	NULL	NULL	gw70_cellbiol_173_2_153_s_91	16636141	A novel and important extension of DeAntoni et al. (2005) was that the kinetochore localization of fluorescently labeled recombinant Mad2 injected into Ptk cells depends on its ability to dimerize with N2'' - Mad2 already bound to Mad1 at the kinetochores.	bind
47481	4	11412	6	NULL	NULL	0	NULL	statement 3	NULL		depends on	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_cellbiol_173_2_153_s_91	16636141	A novel and important extension of DeAntoni et al. (2005) was that the kinetochore localization of fluorescently labeled recombinant Mad2 injected into Ptk cells depends on its ability to dimerize with N2'' - Mad2 already bound to Mad1 at the kinetochores.	bind
50859	1	11415	5	NULL	NULL	NULL	NULL	BTB/POZ transcriptional repressor protein	GP	novel	interacts with					Fanconi anemia group C protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6550_s_590	10938130	A Novel BTB/POZ transcriptional repressor protein interacts with the Fanconi anemia group C protein and PLZF.	bind
50860	2	11415	5	NULL	NULL	NULL	NULL	BTB/POZ transcriptional repressor protein	GP	novel	interacts with					PLZF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_17_6550_s_590	10938130	A Novel BTB/POZ transcriptional repressor protein interacts with the Fanconi anemia group C protein and PLZF.	bind
47483	1	11415	6	NULL	NULL	0	NULL	BTB/POZ transcriptional repressor protein	NULL		interacts with	NULL				Fanconi anemia group C protein	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_17_6550_s_590	10938130	A Novel BTB/POZ transcriptional repressor protein interacts with the Fanconi anemia group C protein and PLZF.	bind
47484	2	11415	6	NULL	NULL	0	NULL	BTB/POZ transcriptional repressor protein	NULL		interacts with	NULL				PLZF	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_17_6550_s_590	10938130	A Novel BTB/POZ transcriptional repressor protein interacts with the Fanconi anemia group C protein and PLZF.	bind
50861	1	11416	5	NULL	NULL	NULL	NULL	factor VIII	GP		bind					von Willebrand factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_23_13826_s_259	7775440	A novel cause of mild/moderate hemophilia A: mutations scattered in the factor VIII C1 domain reduce factor VIII binding to von Willebrand factor.	bind
50862	2	11416	5	NULL	NULL	NULL	NULL	factor VIII	GP	mutant	reduces			C1 domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_23_13826_s_259	7775440	A novel cause of mild/moderate hemophilia A: mutations scattered in the factor VIII C1 domain reduce factor VIII binding to von Willebrand factor.	bind
50863	3	11416	5	NULL	NULL	NULL	NULL	statement 2	Process		causes					hemophilia A	GP	mild/moderate			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_23_13826_s_259	7775440	A novel cause of mild/moderate hemophilia A: mutations scattered in the factor VIII C1 domain reduce factor VIII binding to von Willebrand factor.	bind
47485	1	11416	6	NULL	NULL	0	NULL	factor VIII 	NULL		bind	NULL				von Willebrand factor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_23_13826_s_259	7775440	A novel cause of mild/moderate hemophilia A: mutations scattered in the factor VIII C1 domain reduce factor VIII binding to von Willebrand factor.	bind
47486	2	11416	6	NULL	NULL	0	NULL	factor VIII	NULL	mutant	reduce	NULL		C1 domain		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_23_13826_s_259	7775440	A novel cause of mild/moderate hemophilia A: mutations scattered in the factor VIII C1 domain reduce factor VIII binding to von Willebrand factor.	bind
47487	3	11416	6	NULL	NULL	0	NULL	statement 2	NULL		cause	NULL				hemophilia A	NULL	mild/moderate			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_23_13826_s_259	7775440	A novel cause of mild/moderate hemophilia A: mutations scattered in the factor VIII C1 domain reduce factor VIII binding to von Willebrand factor.	bind
50864	1	11417	5	NULL	NULL	NULL	NULL	MTBP	GP		is a type of					novel cellular protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_67_0_307_s_449	9759491	A Novel Cellular Protein (MTBP) Binds to MDM2 and Induces a G1 Arrest That Is Suppressed by MDM2.	bind
50865	2	11417	5	NULL	NULL	NULL	NULL	MTBP	GP		bind					MDM2	GP				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_67_0_307_s_449	9759491	A Novel Cellular Protein (MTBP) Binds to MDM2 and Induces a G1 Arrest That Is Suppressed by MDM2.	bind
50866	3	11417	5	NULL	NULL	NULL	NULL	statement 2	Process		induce					G1 arrest	Process				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_67_0_307_s_449	9759491	A Novel Cellular Protein (MTBP) Binds to MDM2 and Induces a G1 Arrest That Is Suppressed by MDM2.	bind
50867	4	11417	5	NULL	NULL	NULL	NULL	MDM2	GP		suppress					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_67_0_307_s_449	9759491	A Novel Cellular Protein (MTBP) Binds to MDM2 and Induces a G1 Arrest That Is Suppressed by MDM2.	bind
47488	1	11417	6	NULL	NULL	0	NULL	MTBP	NULL		is a type of	NULL				cellular protein	NULL				NULL		0	NULL	NULL	NULL	gw60_annrevbiochem_67_0_307_s_449	9759491	A Novel Cellular Protein (MTBP) Binds to MDM2 and Induces a G1 Arrest That Is Suppressed by MDM2.	bind
47489	2	11417	6	NULL	NULL	0	NULL	MTBP	NULL		bind	NULL				MDM2	NULL				NULL		0	NULL	NULL	NULL	gw60_annrevbiochem_67_0_307_s_449	9759491	A Novel Cellular Protein (MTBP) Binds to MDM2 and Induces a G1 Arrest That Is Suppressed by MDM2.	bind
47490	3	11417	6	NULL	NULL	0	NULL	statement 2	NULL		induces 	NULL				G1 arrest	NULL				NULL		0	NULL	NULL	NULL	gw60_annrevbiochem_67_0_307_s_449	9759491	A Novel Cellular Protein (MTBP) Binds to MDM2 and Induces a G1 Arrest That Is Suppressed by MDM2.	bind
47491	4	11417	6	10	NULL	0	NULL	MDM2			suppress					statement 3					NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_67_0_307_s_449	9759491	A Novel Cellular Protein (MTBP) Binds to MDM2 and Induces a G1 Arrest That Is Suppressed by MDM2.	bind
50868	1	11418	5	NULL	NULL	NULL	NULL	DNA-binding protein	GP	plant-specific;;zinc-dependent	bind					A/T-rich DNA sequences	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_18_5484_s_511	9736626	A novel class of plant-specific zinc-dependent DNA-binding protein that binds to A/T-rich DNA sequences.	bind
47492	1	11418	6	10	NULL	0	NULL	DNA-binding protein		plant specific;; zinc dependent	bind					A/T-rich DNA sequences					NULL		NULL	NULL	NULL	NULL	gw60_embo_17_18_5484_s_511	9736626	A novel class of plant-specific zinc-dependent DNA-binding protein that binds to A/T-rich DNA sequences.	bind
50869	1	11420	5	NULL	NULL	NULL	NULL	SGT	GP		bind					CSP	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_31_6_987_s_34	11580898	A novel CSP binding partner termed SGT was identified.	bind
47493	1	11420	6	NULL	NULL	0	NULL	SGT	NULL		bind	NULL				CSP	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_31_6_987_s_34	11580898	A novel CSP binding partner termed SGT was identified.	bind
50870	1	11421	5	NULL	NULL	NULL	NULL	SHP1	GP	Rhodobacter sphaeroides	is a type of					novel cytochrome c	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_16050_s_15	10821858	A novel cytochrome  c, which transiently binds O2 during autooxidation, was discovered in the purple phototrophic bacterium  Rhodobacter sphaeroides and was designated SHP1	bind
50871	2	11421	5	NULL	NULL	NULL	NULL	SHP1	GP	Rhodobacter sphaeroides	bind		transiently			O2	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_16050_s_15	10821858	A novel cytochrome  c, which transiently binds O2 during autooxidation, was discovered in the purple phototrophic bacterium  Rhodobacter sphaeroides and was designated SHP1	bind
50872	3	11421	5	NULL	NULL	NULL	NULL	Rhodobacter sphaeroides	Organism		is a type of					purple phototrophic bacterium	Organism				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_16050_s_15	10821858	A novel cytochrome  c, which transiently binds O2 during autooxidation, was discovered in the purple phototrophic bacterium  Rhodobacter sphaeroides and was designated SHP1	bind
54096	4	11421	5	NULL	NULL	NULL	NULL	statement 2	Process		occur during					autooxidation	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_16050_s_15	10821858	A novel cytochrome  c, which transiently binds O2 during autooxidation, was discovered in the purple phototrophic bacterium  Rhodobacter sphaeroides and was designated SHP1	bind
47496	1	11421	6	10	NULL	0	NULL	SHP1		Rhodobacter sphaeroides 	bind		transiently			O2					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_16050_s_15	10821858	A novel cytochrome  c, which transiently binds O2 during autooxidation, was discovered in the purple phototrophic bacterium  Rhodobacter sphaeroides and was designated SHP1	bind
47497	2	11421	6	NULL	NULL	0	NULL	statement 1	NULL		occurs during	NULL				autooxidation	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_16050_s_15	10821858	A novel cytochrome  c, which transiently binds O2 during autooxidation, was discovered in the purple phototrophic bacterium  Rhodobacter sphaeroides and was designated SHP1	bind
47552	3	11421	6	NULL	NULL	0	NULL	Rhodobacter sphaeroides 	NULL		is a type of	NULL				purple photographic bacterium	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_16050_s_15	10821858	A novel cytochrome  c, which transiently binds O2 during autooxidation, was discovered in the purple phototrophic bacterium  Rhodobacter sphaeroides and was designated SHP1	bind
47553	4	11421	6	NULL	NULL	0	NULL	SHP1	NULL		is a type of	NULL				cytochrome c	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_16050_s_15	10821858	A novel cytochrome  c, which transiently binds O2 during autooxidation, was discovered in the purple phototrophic bacterium  Rhodobacter sphaeroides and was designated SHP1	bind
50873	1	11422	5	NULL	NULL	NULL	NULL	CIS	GP		is a type of					cytokine-indicible gene	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_12_3299_s_356	9843570	A novel cytokine-indicible gene CIS encodes an SH2-containing protein that binds to tyrosine-phosphorylated interleukin 3 and erythropoietin receptors.	bind
50874	2	11422	5	NULL	NULL	NULL	NULL	CIS	GP		encodes					SH2-containing protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_12_3299_s_356	9843570	A novel cytokine-indicible gene CIS encodes an SH2-containing protein that binds to tyrosine-phosphorylated interleukin 3 and erythropoietin receptors.	bind
50875	3	11422	5	NULL	NULL	NULL	NULL	statement 2	Process		bind					interleukin 3	GP	phosphorylated	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_12_3299_s_356	9843570	A novel cytokine-indicible gene CIS encodes an SH2-containing protein that binds to tyrosine-phosphorylated interleukin 3 and erythropoietin receptors.	bind
50876	4	11422	5	NULL	NULL	NULL	NULL	statement 2	Process		bind					erythropoietin receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_12_3299_s_356	9843570	A novel cytokine-indicible gene CIS encodes an SH2-containing protein that binds to tyrosine-phosphorylated interleukin 3 and erythropoietin receptors.	bind
47554	1	11422	6	NULL	NULL	0	NULL	CIS	NULL		is induced by	NULL				cytokine	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_9_12_3299_s_356	9843570	A novel cytokine-indicible gene CIS encodes an SH2-containing protein that binds to tyrosine-phosphorylated interleukin 3 and erythropoietin receptors.	bind
47555	2	11422	6	NULL	NULL	0	NULL	CIS	NULL		encodes	NULL				SH2-containing protein	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_9_12_3299_s_356	9843570	A novel cytokine-indicible gene CIS encodes an SH2-containing protein that binds to tyrosine-phosphorylated interleukin 3 and erythropoietin receptors.	bind
47556	3	11422	6	NULL	NULL	0	NULL	statement 2	NULL		bind	NULL				interleukin 3	NULL	phosphorylated	tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_9_12_3299_s_356	9843570	A novel cytokine-indicible gene CIS encodes an SH2-containing protein that binds to tyrosine-phosphorylated interleukin 3 and erythropoietin receptors.	bind
47557	4	11422	6	NULL	NULL	0	NULL	statement 2	NULL		bind	NULL				erythropoietin receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_9_12_3299_s_356	9843570	A novel cytokine-indicible gene CIS encodes an SH2-containing protein that binds to tyrosine-phosphorylated interleukin 3 and erythropoietin receptors.	bind
50877	1	11432	5	NULL	NULL	NULL	NULL	Rheb	GP		bind					mTOR effector	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_23433_s_88	15878852	A novel feature of the binding of Rheb to its effector mTOR, and one that contrasts with the interaction of other Ras-like GTPases with their known effectors, is that the Rheb-mTOR interaction does not require Rheb GTP charging ( ).	bind
50878	2	11432	5	NULL	NULL	NULL	NULL	statement 1	Process		does not require					Rheb GTP	GP	charging of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_23433_s_88	15878852	A novel feature of the binding of Rheb to its effector mTOR, and one that contrasts with the interaction of other Ras-like GTPases with their known effectors, is that the Rheb-mTOR interaction does not require Rheb GTP charging ( ).	bind
47816	1	11432	6	NULL	NULL	0	NULL	Rheb	NULL		bind	NULL				mTOR effector	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_25_23433_s_88	15878852	A novel feature of the binding of Rheb to its effector mTOR, and one that contrasts with the interaction of other Ras-like GTPases with their known effectors, is that the Rheb-mTOR interaction does not require Rheb GTP charging ( ).	bind
47817	2	11432	6	NULL	NULL	0	NULL	statement 1	NULL		does not require	NULL				Rheb G GTP	NULL	charging of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_25_23433_s_88	15878852	A novel feature of the binding of Rheb to its effector mTOR, and one that contrasts with the interaction of other Ras-like GTPases with their known effectors, is that the Rheb-mTOR interaction does not require Rheb GTP charging ( ).	bind
50879	1	11433	5	NULL	NULL	NULL	NULL	MAPK	GP		regulates		differentially			GATA-4	GP	binding activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_16_13752_s_281	11827958	A novel finding in our studies is the differential regulation of GATA-4 binding activity by MAPKs.	bind
47558	1	11433	6	NULL	NULL	0	NULL	MAPK	NULL		regulates	NULL	differentially			GATA-4	NULL	binding activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_16_13752_s_281	11827958	A novel finding in our studies is the differential regulation of GATA-4 binding activity by MAPKs.	bind
50880	1	11434	5	NULL	NULL	NULL	NULL	grB	GP		bind					serglycin	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_2_623_s_322	16280358	A novel finding is that this is the critical mechanism of uptake when grB is bound to serglycin.	bind
47559	1	11434	6	NULL	NULL	0	NULL	grB	NULL		bind	NULL				serglycin	NULL				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_2_623_s_322	16280358	A novel finding is that this is the critical mechanism of uptake when grB is bound to serglycin.	bind
50881	1	11437	5	NULL	NULL	NULL	NULL	VEGF	GP		bind					VEGF receptor-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_2_171_s_417	12887919	A novel function for tissue inhibitor of metalloproteinases-3 (TIMP3): inhibition of angiogenesis by blockage of VEGF binding to VEGF receptor-2.	bind
50882	2	11437	5	NULL	NULL	NULL	NULL	TIMP3	GP		is					tissue inhibitor of metalloproteinases-3	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_2_171_s_417	12887919	A novel function for tissue inhibitor of metalloproteinases-3 (TIMP3): inhibition of angiogenesis by blockage of VEGF binding to VEGF receptor-2.	bind
50883	3	11437	5	NULL	NULL	NULL	NULL	TIMP3	GP		inhibits					angiogenesis	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_2_171_s_417	12887919	A novel function for tissue inhibitor of metalloproteinases-3 (TIMP3): inhibition of angiogenesis by blockage of VEGF binding to VEGF receptor-2.	bind
50884	4	11437	5	NULL	NULL	NULL	NULL	TIMP3	GP		blocks					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_2_171_s_417	12887919	A novel function for tissue inhibitor of metalloproteinases-3 (TIMP3): inhibition of angiogenesis by blockage of VEGF binding to VEGF receptor-2.	bind
50885	5	11437	5	NULL	NULL	NULL	NULL	statement 4	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_114_2_171_s_417	12887919	A novel function for tissue inhibitor of metalloproteinases-3 (TIMP3): inhibition of angiogenesis by blockage of VEGF binding to VEGF receptor-2.	bind
47561	1	11437	6	NULL	NULL	0	NULL	VEGF	NULL		bind	NULL				VEGF receptor-2	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_114_2_171_s_417	12887919	A novel function for tissue inhibitor of metalloproteinases-3 (TIMP3): inhibition of angiogenesis by blockage of VEGF binding to VEGF receptor-2.	bind
47562	2	11437	6	NULL	NULL	0	NULL	TIMP-3	NULL		blocks	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_114_2_171_s_417	12887919	A novel function for tissue inhibitor of metalloproteinases-3 (TIMP3): inhibition of angiogenesis by blockage of VEGF binding to VEGF receptor-2.	bind
47563	3	11437	6	NULL	NULL	0	NULL	statement 2	NULL		inhibits	NULL				angiogenesis	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_114_2_171_s_417	12887919	A novel function for tissue inhibitor of metalloproteinases-3 (TIMP3): inhibition of angiogenesis by blockage of VEGF binding to VEGF receptor-2.	bind
47564	4	11437	6	NULL	NULL	0	NULL	TIMP3	NULL		is	NULL				tissue inhibitor of metalloproteinases-3	NULL				NULL		0	NULL	NULL	NULL	gw60_cell_114_2_171_s_417	12887919	A novel function for tissue inhibitor of metalloproteinases-3 (TIMP3): inhibition of angiogenesis by blockage of VEGF binding to VEGF receptor-2.	bind
54097	5	11437	6	10	NULL	0	NULL	statement 2			leads to					statement 3					NULL		0	NULL	NULL	NULL	gw60_cell_114_2_171_s_417	12887919	A novel function for tissue inhibitor of metalloproteinases-3 (TIMP3): inhibition of angiogenesis by blockage of VEGF binding to VEGF receptor-2.	bind
50897	1	11439	5	NULL	NULL	NULL	NULL	frizzled wnt receptor gene	GP	human	is homologous to					frizzled wnt receptor gene	GP	Drosophila			NULL		NULL	NULL	NULL	NULL	gw70_annurevgenomicshum_1_0_461_s_1047	null	A novel human homologue of the  Drosophila frizzled wnt receptor gene binds wingless protein and is in the Williams syndrome  deletion at 7q11.	bind
50898	2	11439	5	NULL	NULL	NULL	NULL	frizzled wnt receptor gene	GP	human	bind					wingless protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevgenomicshum_1_0_461_s_1047	null	A novel human homologue of the  Drosophila frizzled wnt receptor gene binds wingless protein and is in the Williams syndrome  deletion at 7q11.	bind
50899	3	11439	5	NULL	NULL	NULL	NULL			deletion of	leads to				7q11	Williams syndrome	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw70_annurevgenomicshum_1_0_461_s_1047	null	A novel human homologue of the  Drosophila frizzled wnt receptor gene binds wingless protein and is in the Williams syndrome  deletion at 7q11.	bind
47565	1	11439	6	10	NULL	0	NULL	frizzled wnt receptor gene		human	is homologous to					frizzled wnt receptor gene		Drosophila			NULL		NULL	NULL	NULL	NULL	gw70_annurevgenomicshum_1_0_461_s_1047	null	A novel human homologue of the  Drosophila frizzled wnt receptor gene binds wingless protein and is in the Williams syndrome  deletion at 7q11.	bind
47566	2	11439	6	10	NULL	0	NULL	frizzled wnt receptor gene		human	bind					wingless protein					NULL		NULL	NULL	NULL	NULL	gw70_annurevgenomicshum_1_0_461_s_1047	null	A novel human homologue of the  Drosophila frizzled wnt receptor gene binds wingless protein and is in the Williams syndrome  deletion at 7q11.	bind
47567	3	11439	6	10	NULL	0	NULL			deletion of	leads to				7q11	Williams syndrome					NULL		NULL	NULL	NULL	NULL	gw70_annurevgenomicshum_1_0_461_s_1047	null	A novel human homologue of the  Drosophila frizzled wnt receptor gene binds wingless protein and is in the Williams syndrome  deletion at 7q11.	bind
50900	1	11443	5	NULL	NULL	NULL	NULL	Neisseria gonorrhoeae	Organism		is a type of					pathogen	Organism				NULL		NULL	NULL	NULL	NULL	gw60_vetmicrobiol_94_2_131_s_9	12781481	A novel mechanism for microbial exploitation of host factors was described in  Neisseria gonorrhoeae in which this pathogen bound heparin sulfate that directed the binding of vitronectin, which ultimately was used as a bridge to attach to host surfaces (  Duensing and Van Putten, 1998).	bind
50901	2	11443	5	NULL	NULL	NULL	NULL	Neisseria gonorrhoeae	Organism		bind					heparin sulfate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_vetmicrobiol_94_2_131_s_9	12781481	A novel mechanism for microbial exploitation of host factors was described in  Neisseria gonorrhoeae in which this pathogen bound heparin sulfate that directed the binding of vitronectin, which ultimately was used as a bridge to attach to host surfaces (  Duensing and Van Putten, 1998).	bind
50902	3	11443	5	NULL	NULL	NULL	NULL	statement 1	Process		directs					vitronectin	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_vetmicrobiol_94_2_131_s_9	12781481	A novel mechanism for microbial exploitation of host factors was described in  Neisseria gonorrhoeae in which this pathogen bound heparin sulfate that directed the binding of vitronectin, which ultimately was used as a bridge to attach to host surfaces (  Duensing and Van Putten, 1998).	bind
47820	1	11443	6	NULL	NULL	0	NULL	Neisseria gonorrhoeae	NULL		bind	NULL				heparin sulfate	NULL				NULL		0	NULL	NULL	NULL	gw60_vetmicrobiol_94_2_131_s_9	12781481	A novel mechanism for microbial exploitation of host factors was described in  Neisseria gonorrhoeae in which this pathogen bound heparin sulfate that directed the binding of vitronectin, which ultimately was used as a bridge to attach to host surfaces (  Duensing and Van Putten, 1998).	bind
47821	2	11443	6	NULL	NULL	0	NULL	statement 1	NULL		directed 	NULL				vitronectin	NULL	binding of 			NULL		0	NULL	NULL	NULL	gw60_vetmicrobiol_94_2_131_s_9	12781481	A novel mechanism for microbial exploitation of host factors was described in  Neisseria gonorrhoeae in which this pathogen bound heparin sulfate that directed the binding of vitronectin, which ultimately was used as a bridge to attach to host surfaces (  Duensing and Van Putten, 1998).	bind
58568	3	11443	6	10	NULL	0	NULL	Neisseria gonorrhoeae			is a type of					pathogen					NULL		0	NULL	NULL	NULL	gw60_vetmicrobiol_94_2_131_s_9	12781481	A novel mechanism for microbial exploitation of host factors was described in  Neisseria gonorrhoeae in which this pathogen bound heparin sulfate that directed the binding of vitronectin, which ultimately was used as a bridge to attach to host surfaces (  Duensing and Van Putten, 1998).	bind
50903	1	11445	5	NULL	NULL	NULL	NULL	S-nitrosoglutathione	Chemical		is a type of					NO releaser	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_11_3486_s_446	10348862	A novel mechanism for upregulation of the  Escherichia coli K-12  hmp (flavohaemoglobin) gene by the 'NO releaser'', S-nitrosoglutathione: nitrosation of homocysteine and modulation of MetR binding to the gly  hmp intergenic region.	bind
50904	2	11445	5	NULL	NULL	NULL	NULL	S-nitrosoglutathione	GP		upregulates					hmp gene	GP	Escherichia coli K-12			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_11_3486_s_446	10348862	A novel mechanism for upregulation of the  Escherichia coli K-12  hmp (flavohaemoglobin) gene by the 'NO releaser'', S-nitrosoglutathione: nitrosation of homocysteine and modulation of MetR binding to the gly  hmp intergenic region.	bind
50905	3	11445	5	NULL	NULL	NULL	NULL	hmp	GP		is					flavohaemoglobin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_11_3486_s_446	10348862	A novel mechanism for upregulation of the  Escherichia coli K-12  hmp (flavohaemoglobin) gene by the 'NO releaser'', S-nitrosoglutathione: nitrosation of homocysteine and modulation of MetR binding to the gly  hmp intergenic region.	bind
50907	4	11445	5	NULL	NULL	NULL	NULL	MetR	GP		bind									gly hmp intergenic region	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_11_3486_s_446	10348862	A novel mechanism for upregulation of the  Escherichia coli K-12  hmp (flavohaemoglobin) gene by the 'NO releaser'', S-nitrosoglutathione: nitrosation of homocysteine and modulation of MetR binding to the gly  hmp intergenic region.	bind
47846	1	11445	6	NULL	NULL	0	NULL	MetR	NULL		bind	NULL					NULL			gly hmp intergenic region	NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_11_3486_s_446	10348862	A novel mechanism for upregulation of the  Escherichia coli K-12  hmp (flavohaemoglobin) gene by the 'NO releaser'', S-nitrosoglutathione: nitrosation of homocysteine and modulation of MetR binding to the gly  hmp intergenic region.	bind
47847	2	11445	6	NULL	NULL	0	NULL	S-nitrosoglutathione	NULL		is a type of	NULL				NO releaser	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_11_3486_s_446	10348862	A novel mechanism for upregulation of the  Escherichia coli K-12  hmp (flavohaemoglobin) gene by the 'NO releaser'', S-nitrosoglutathione: nitrosation of homocysteine and modulation of MetR binding to the gly  hmp intergenic region.	bind
47860	3	11445	6	NULL	NULL	0	NULL	S-nitrosoglutathione	NULL		upregulates	NULL				hmp gene	NULL	Escherichia coli K-12			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_11_3486_s_446	10348862	A novel mechanism for upregulation of the  Escherichia coli K-12  hmp (flavohaemoglobin) gene by the 'NO releaser'', S-nitrosoglutathione: nitrosation of homocysteine and modulation of MetR binding to the gly  hmp intergenic region.	bind
47861	4	11445	6	NULL	NULL	0	NULL	hmp	NULL		is	NULL				flavohaemoglobin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_11_3486_s_446	10348862	A novel mechanism for upregulation of the  Escherichia coli K-12  hmp (flavohaemoglobin) gene by the 'NO releaser'', S-nitrosoglutathione: nitrosation of homocysteine and modulation of MetR binding to the gly  hmp intergenic region.	bind
50909	1	11447	5	NULL	NULL	NULL	NULL	SHPS-1	GP		is a type of					membrane glycoprotein	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_17_0_875_s_917	10358776	A novel membrane glycoprotein, SHPS-1, that  binds the SH2-domain-containing protein tyrosine phosphatase SHP-2 in response to  mitogens and cell adhesion.	bind
50910	2	11447	5	NULL	NULL	NULL	NULL	SHPS-1	GP		bind					SHP-2	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_17_0_875_s_917	10358776	A novel membrane glycoprotein, SHPS-1, that  binds the SH2-domain-containing protein tyrosine phosphatase SHP-2 in response to  mitogens and cell adhesion.	bind
50911	3	11447	5	NULL	NULL	NULL	NULL	SHP-2	GP		is					SH2-domain-containing protein tyrosine phosphatase	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_17_0_875_s_917	10358776	A novel membrane glycoprotein, SHPS-1, that  binds the SH2-domain-containing protein tyrosine phosphatase SHP-2 in response to  mitogens and cell adhesion.	bind
50912	4	11447	5	NULL	NULL	NULL	NULL	statement 2	Process		in response to					mitogens	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_17_0_875_s_917	10358776	A novel membrane glycoprotein, SHPS-1, that  binds the SH2-domain-containing protein tyrosine phosphatase SHP-2 in response to  mitogens and cell adhesion.	bind
50913	5	11447	5	NULL	NULL	NULL	NULL	statement 2	Process		in response to					cell adhesion	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_17_0_875_s_917	10358776	A novel membrane glycoprotein, SHPS-1, that  binds the SH2-domain-containing protein tyrosine phosphatase SHP-2 in response to  mitogens and cell adhesion.	bind
47568	1	11447	6	10	NULL	0	NULL	SHPS-1			is a type of					membrane glycoprotein					NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_17_0_875_s_917	10358776	A novel membrane glycoprotein, SHPS-1, that  binds the SH2-domain-containing protein tyrosine phosphatase SHP-2 in response to  mitogens and cell adhesion.	bind
47569	2	11447	6	NULL	NULL	0	NULL	SHP-2	NULL		is	NULL				SH2-domain-containing protein tyrosine phosphatase	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_875_s_917	10358776	A novel membrane glycoprotein, SHPS-1, that  binds the SH2-domain-containing protein tyrosine phosphatase SHP-2 in response to  mitogens and cell adhesion.	bind
47570	3	11447	6	NULL	NULL	0	NULL	SHPS-1	NULL		bind	NULL				SHP-2	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_875_s_917	10358776	A novel membrane glycoprotein, SHPS-1, that  binds the SH2-domain-containing protein tyrosine phosphatase SHP-2 in response to  mitogens and cell adhesion.	bind
47571	4	11447	6	NULL	NULL	0	NULL	statement 3	NULL		occurs in response to	NULL				mitogen	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_875_s_917	10358776	A novel membrane glycoprotein, SHPS-1, that  binds the SH2-domain-containing protein tyrosine phosphatase SHP-2 in response to  mitogens and cell adhesion.	bind
47572	5	11447	6	NULL	NULL	0	NULL	statement 3	NULL		occurs in response to	NULL				cell adhesion	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_875_s_917	10358776	A novel membrane glycoprotein, SHPS-1, that  binds the SH2-domain-containing protein tyrosine phosphatase SHP-2 in response to  mitogens and cell adhesion.	bind
50914	1	11450	5	NULL	NULL	NULL	NULL	SW-480	Cell		is a type of					human colon carcinoma cell line	Cell				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_18_6837_s_452	10958680	A novel mitogenic signaling pathway of bradykinin in the human colon carcinoma cell line SW-480 involves sequential activation of a Gq/11 protein, phosphatidylinositol 3-kinase beta, and [[ protein kinase C.  J. Biol. Chem.  273 ]] :32016-32022 [Abstract/ull Text].	bind
50915	2	11450	5	NULL	NULL	NULL	NULL	bradykinin	GP	mitogenic signaling pathway of	involves					Gq/11 protein	GP	sequential activation of			NULL	SW-480 cell line	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_18_6837_s_452	10958680	A novel mitogenic signaling pathway of bradykinin in the human colon carcinoma cell line SW-480 involves sequential activation of a Gq/11 protein, phosphatidylinositol 3-kinase beta, and [[ protein kinase C.  J. Biol. Chem.  273 ]] :32016-32022 [Abstract/ull Text].	bind
50916	3	11450	5	NULL	NULL	NULL	NULL	bradykinin	GP	mitogenic signaling pathway of	involves					phosphatidylinositol 3-kinase beta	GP	sequential activation of			NULL	SW-480 cell line	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_18_6837_s_452	10958680	A novel mitogenic signaling pathway of bradykinin in the human colon carcinoma cell line SW-480 involves sequential activation of a Gq/11 protein, phosphatidylinositol 3-kinase beta, and [[ protein kinase C.  J. Biol. Chem.  273 ]] :32016-32022 [Abstract/ull Text].	bind
50917	4	11450	5	NULL	NULL	NULL	NULL	bradykinin	GP	mitogenic signaling pathway of	involves					protein kinase C	GP	sequential activation of			NULL	SW-480 cell line	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_18_6837_s_452	10958680	A novel mitogenic signaling pathway of bradykinin in the human colon carcinoma cell line SW-480 involves sequential activation of a Gq/11 protein, phosphatidylinositol 3-kinase beta, and [[ protein kinase C.  J. Biol. Chem.  273 ]] :32016-32022 [Abstract/ull Text].	bind
47573	1	11450	6	10	NULL	0	NULL	SW-480			is a type of					human colon carcinoma cell line					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_18_6837_s_452	10958680	A novel mitogenic signaling pathway of bradykinin in the human colon carcinoma cell line SW-480 involves sequential activation of a Gq/11 protein, phosphatidylinositol 3-kinase beta, and [[ protein kinase C.  J. Biol. Chem.  273 ]] :32016-32022 [Abstract/ull Text].	bind
47689	2	11450	6	10	NULL	0	NULL	bradykinin 		mitogenic signaling pathway of	involves					Gq/11 protein		sequential activation of			NULL	SW-480 cell line	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_18_6837_s_452	10958680	A novel mitogenic signaling pathway of bradykinin in the human colon carcinoma cell line SW-480 involves sequential activation of a Gq/11 protein, phosphatidylinositol 3-kinase beta, and [[ protein kinase C.  J. Biol. Chem.  273 ]] :32016-32022 [Abstract/ull Text].	bind
47690	3	11450	6	10	NULL	0	NULL	bradykinin		mitogenic signaling pathway of	involves					phosphatidylinositol 3-kinase beta		sequential activation of			NULL	SW-480 cell line	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_18_6837_s_452	10958680	A novel mitogenic signaling pathway of bradykinin in the human colon carcinoma cell line SW-480 involves sequential activation of a Gq/11 protein, phosphatidylinositol 3-kinase beta, and [[ protein kinase C.  J. Biol. Chem.  273 ]] :32016-32022 [Abstract/ull Text].	bind
47691	4	11450	6	10	NULL	0	NULL	bradykinin 		mitogenic signaling pathway of	involves					protein kinase C		sequential activation of			NULL	SW-480 cell line	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_18_6837_s_452	10958680	A novel mitogenic signaling pathway of bradykinin in the human colon carcinoma cell line SW-480 involves sequential activation of a Gq/11 protein, phosphatidylinositol 3-kinase beta, and [[ protein kinase C.  J. Biol. Chem.  273 ]] :32016-32022 [Abstract/ull Text].	bind
50918	1	11451	5	NULL	NULL	NULL	NULL	MIBP	GP		is					muscle-specific beta1 integrin binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_150_4_861_s_332	10953009	A novel muscle-specific beta1 integrin binding protein (MIBP) that modulates myogenic differentiation.	bind
50919	2	11451	5	NULL	NULL	NULL	NULL	MIBP	GP		modulates					myogenic differentiation	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_150_4_861_s_332	10953009	A novel muscle-specific beta1 integrin binding protein (MIBP) that modulates myogenic differentiation.	bind
47692	1	11451	6	NULL	NULL	0	NULL	MIBP	NULL		modulates	NULL				myogenic differentiation	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_150_4_861_s_332	10953009	A novel muscle-specific beta1 integrin binding protein (MIBP) that modulates myogenic differentiation.	bind
47693	2	11451	6	NULL	NULL	0	NULL	MIBP	NULL		is	NULL				muscle-specific beta1 integrin binding protein	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_150_4_861_s_332	10953009	A novel muscle-specific beta1 integrin binding protein (MIBP) that modulates myogenic differentiation.	bind
50920	1	11452	5	NULL	NULL	NULL	NULL	cardiac ryanodine receptor gene	GP	human;;mutant	causes			R2401H in FKBP12.6 binding region		catecholaminergic polymorphic ventricular tachycardia	MedicalFinding				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_int-j-cardiol_99_2_15749201_s_1	15749201	A novel mutation in FKBP12.6 binding region of the human cardiac ryanodine receptor gene (R2401H) in a Japanese patient with catecholaminergic polymorphic ventricular tachycardia..	bind
47694	1	11452	6	NULL	NULL	0	NULL	catecholaminergic polymorphic ventricular tachycardia	NULL		involves	NULL				cardiac ryanodine receptor gene	NULL	mutation of	R2401 in FKBP12.6 binding region		NULL		0	NULL	NULL	NULL	abs-batch0720-0739_int-j-cardiol_99_2_15749201_s_1	15749201	A novel mutation in FKBP12.6 binding region of the human cardiac ryanodine receptor gene (R2401H) in a Japanese patient with catecholaminergic polymorphic ventricular tachycardia..	bind
50921	1	11453	5	NULL	NULL	NULL	NULL	N-WASP	GP		is					neural Wiskott-Aldrich syndrome protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_13_7_534_s_487	12676083	A novel neural Wiskott-Aldrich syndrome protein (N-WASP) binding protein, WISH, induces Arp2/3 complex activation independent of Cdc42.	bind
50922	2	11453	5	NULL	NULL	NULL	NULL	WISH	GP		bind					N-WASP	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_13_7_534_s_487	12676083	A novel neural Wiskott-Aldrich syndrome protein (N-WASP) binding protein, WISH, induces Arp2/3 complex activation independent of Cdc42.	bind
50923	3	11453	5	NULL	NULL	NULL	NULL	WISH	GP		induces					Arp2/3 complex	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_13_7_534_s_487	12676083	A novel neural Wiskott-Aldrich syndrome protein (N-WASP) binding protein, WISH, induces Arp2/3 complex activation independent of Cdc42.	bind
50924	4	11453	5	NULL	NULL	NULL	NULL	statement 3	Process		is independent of					Cdc42	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_13_7_534_s_487	12676083	A novel neural Wiskott-Aldrich syndrome protein (N-WASP) binding protein, WISH, induces Arp2/3 complex activation independent of Cdc42.	bind
47695	1	11453	6	NULL	NULL	0	NULL	WISH	NULL		bind	NULL				N-WASP	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_13_7_534_s_487	12676083	A novel neural Wiskott-Aldrich syndrome protein (N-WASP) binding protein, WISH, induces Arp2/3 complex activation independent of Cdc42.	bind
47696	2	11453	6	NULL	NULL	0	NULL	N-WASP	NULL		is	NULL				neural Wiskott-Aldrich syndrome protein	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_13_7_534_s_487	12676083	A novel neural Wiskott-Aldrich syndrome protein (N-WASP) binding protein, WISH, induces Arp2/3 complex activation independent of Cdc42.	bind
47697	3	11453	6	NULL	NULL	0	NULL	WISH	NULL		induces	NULL				Arp2/3 complex	NULL	activation of			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_13_7_534_s_487	12676083	A novel neural Wiskott-Aldrich syndrome protein (N-WASP) binding protein, WISH, induces Arp2/3 complex activation independent of Cdc42.	bind
47698	4	11453	6	NULL	NULL	0	NULL	statement 3	NULL		is independent of	NULL				Cdc42	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_13_7_534_s_487	12676083	A novel neural Wiskott-Aldrich syndrome protein (N-WASP) binding protein, WISH, induces Arp2/3 complex activation independent of Cdc42.	bind
50926	1	11454	5	NULL	NULL	NULL	NULL	Noc/OFQ	GP		bind					receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_303_1_424_s_150	12235279	A novel nonpeptide Noc/OFQ antagonist JTC-801 was recently synthesized (Shinkai et al., 2000  ) and shown to inhibit [3]Noc/OFQ binding to the receptor ( Ki = 44.5 nM) and antagonize the suppression of Noc/OFQ on forskolin-induced cAMP formation (IC50 = 2.58 muM) in HeLa cells expressing human Noc/OFQ receptor (Yamada et al., 2002  ).	bind
50927	2	11454	5	NULL	NULL	NULL	NULL	JTC-801	Chemical		is an antagonist of					Noc/OFQ	GP				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_303_1_424_s_150	12235279	A novel nonpeptide Noc/OFQ antagonist JTC-801 was recently synthesized (Shinkai et al., 2000  ) and shown to inhibit [3]Noc/OFQ binding to the receptor ( Ki = 44.5 nM) and antagonize the suppression of Noc/OFQ on forskolin-induced cAMP formation (IC50 = 2.58 muM) in HeLa cells expressing human Noc/OFQ receptor (Yamada et al., 2002  ).	bind
50928	3	11454	5	NULL	NULL	NULL	NULL	JTC-801	Chemical		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_303_1_424_s_150	12235279	A novel nonpeptide Noc/OFQ antagonist JTC-801 was recently synthesized (Shinkai et al., 2000  ) and shown to inhibit [3]Noc/OFQ binding to the receptor ( Ki = 44.5 nM) and antagonize the suppression of Noc/OFQ on forskolin-induced cAMP formation (IC50 = 2.58 muM) in HeLa cells expressing human Noc/OFQ receptor (Yamada et al., 2002  ).	bind
50929	4	11454	5	NULL	NULL	NULL	NULL	forskolin	Chemical		induce					cAMP	Chemical	formation of			NULL	HeLa cells expressing human Noc/OFQ receptor	NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_303_1_424_s_150	12235279	A novel nonpeptide Noc/OFQ antagonist JTC-801 was recently synthesized (Shinkai et al., 2000  ) and shown to inhibit [3]Noc/OFQ binding to the receptor ( Ki = 44.5 nM) and antagonize the suppression of Noc/OFQ on forskolin-induced cAMP formation (IC50 = 2.58 muM) in HeLa cells expressing human Noc/OFQ receptor (Yamada et al., 2002  ).	bind
50930	5	11454	5	NULL	NULL	NULL	NULL	Noc/OFQ	GP		is supressed by					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_303_1_424_s_150	12235279	A novel nonpeptide Noc/OFQ antagonist JTC-801 was recently synthesized (Shinkai et al., 2000  ) and shown to inhibit [3]Noc/OFQ binding to the receptor ( Ki = 44.5 nM) and antagonize the suppression of Noc/OFQ on forskolin-induced cAMP formation (IC50 = 2.58 muM) in HeLa cells expressing human Noc/OFQ receptor (Yamada et al., 2002  ).	bind
50931	6	11454	5	NULL	NULL	NULL	NULL	JTC-801	Chemical		antagonize					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_303_1_424_s_150	12235279	A novel nonpeptide Noc/OFQ antagonist JTC-801 was recently synthesized (Shinkai et al., 2000  ) and shown to inhibit [3]Noc/OFQ binding to the receptor ( Ki = 44.5 nM) and antagonize the suppression of Noc/OFQ on forskolin-induced cAMP formation (IC50 = 2.58 muM) in HeLa cells expressing human Noc/OFQ receptor (Yamada et al., 2002  ).	bind
47699	1	11454	6	NULL	NULL	0	NULL	Noc/OFQ	NULL		bind	NULL				receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_303_1_424_s_150	12235279	A novel nonpeptide Noc/OFQ antagonist JTC-801 was recently synthesized (Shinkai et al., 2000  ) and shown to inhibit [3]Noc/OFQ binding to the receptor ( Ki = 44.5 nM) and antagonize the suppression of Noc/OFQ on forskolin-induced cAMP formation (IC50 = 2.58 muM) in HeLa cells expressing human Noc/OFQ receptor (Yamada et al., 2002  ).	bind
47700	2	11454	6	10	NULL	0	NULL	JTC-801			is an antagonist of					Noc/OFQ 					NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_303_1_424_s_150	12235279	A novel nonpeptide Noc/OFQ antagonist JTC-801 was recently synthesized (Shinkai et al., 2000  ) and shown to inhibit [3]Noc/OFQ binding to the receptor ( Ki = 44.5 nM) and antagonize the suppression of Noc/OFQ on forskolin-induced cAMP formation (IC50 = 2.58 muM) in HeLa cells expressing human Noc/OFQ receptor (Yamada et al., 2002  ).	bind
47701	3	11454	6	NULL	NULL	0	NULL	JTC-801	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_303_1_424_s_150	12235279	A novel nonpeptide Noc/OFQ antagonist JTC-801 was recently synthesized (Shinkai et al., 2000  ) and shown to inhibit [3]Noc/OFQ binding to the receptor ( Ki = 44.5 nM) and antagonize the suppression of Noc/OFQ on forskolin-induced cAMP formation (IC50 = 2.58 muM) in HeLa cells expressing human Noc/OFQ receptor (Yamada et al., 2002  ).	bind
47702	4	11454	6	NULL	NULL	0	NULL	forskolin	NULL		induces	NULL				cAMP	NULL	formation of			NULL	HeLa cells expressing human Noc/OFQ receptor	0	NULL	NULL	NULL	gw60_jpharmacolexpther_303_1_424_s_150	12235279	A novel nonpeptide Noc/OFQ antagonist JTC-801 was recently synthesized (Shinkai et al., 2000  ) and shown to inhibit [3]Noc/OFQ binding to the receptor ( Ki = 44.5 nM) and antagonize the suppression of Noc/OFQ on forskolin-induced cAMP formation (IC50 = 2.58 muM) in HeLa cells expressing human Noc/OFQ receptor (Yamada et al., 2002  ).	bind
47703	5	11454	6	NULL	NULL	0	NULL	Noc/OFQ	NULL		suppresses	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_303_1_424_s_150	12235279	A novel nonpeptide Noc/OFQ antagonist JTC-801 was recently synthesized (Shinkai et al., 2000  ) and shown to inhibit [3]Noc/OFQ binding to the receptor ( Ki = 44.5 nM) and antagonize the suppression of Noc/OFQ on forskolin-induced cAMP formation (IC50 = 2.58 muM) in HeLa cells expressing human Noc/OFQ receptor (Yamada et al., 2002  ).	bind
47704	6	11454	6	10	NULL	0	NULL	JTC-801			antagonizes					statement 5					NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_303_1_424_s_150	12235279	A novel nonpeptide Noc/OFQ antagonist JTC-801 was recently synthesized (Shinkai et al., 2000  ) and shown to inhibit [3]Noc/OFQ binding to the receptor ( Ki = 44.5 nM) and antagonize the suppression of Noc/OFQ on forskolin-induced cAMP formation (IC50 = 2.58 muM) in HeLa cells expressing human Noc/OFQ receptor (Yamada et al., 2002  ).	bind
50932	1	11456	5	NULL	NULL	NULL	NULL	ost	GP		is a type of					oncogene	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_4986_s_376	9710582	A novel oncogene, ost, encodes a guanine nucleotide exchange factor that potentially links Rho and Rac signaling pathways.	bind
50933	2	11456	5	NULL	NULL	NULL	NULL	ost	GP		encodes					guanine nucleotide exchange factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_4986_s_376	9710582	A novel oncogene, ost, encodes a guanine nucleotide exchange factor that potentially links Rho and Rac signaling pathways.	bind
50934	3	11456	5	NULL	NULL	NULL	NULL	Rho signaling pathway	Process		is linked to					Rac signaling pathway	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_4986_s_376	9710582	A novel oncogene, ost, encodes a guanine nucleotide exchange factor that potentially links Rho and Rac signaling pathways.	bind
50935	4	11456	5	NULL	NULL	NULL	NULL	statement 2	Process		is required for					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_4986_s_376	9710582	A novel oncogene, ost, encodes a guanine nucleotide exchange factor that potentially links Rho and Rac signaling pathways.	bind
47705	1	11456	6	10	NULL	0	NULL	ost			encodes 					guanine nucleotide exchange factor					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_4986_s_376	9710582	A novel oncogene, ost, encodes a guanine nucleotide exchange factor that potentially links Rho and Rac signaling pathways.	bind
47706	2	11456	6	NULL	NULL	0	NULL	Rho signaling pathway	NULL		is linked to	NULL				Rac signaling pathway	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_9_4986_s_376	9710582	A novel oncogene, ost, encodes a guanine nucleotide exchange factor that potentially links Rho and Rac signaling pathways.	bind
47707	3	11456	6	10	NULL	0	NULL	guanine nucleotide exchange factor			is required for					statement 2					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_4986_s_376	9710582	A novel oncogene, ost, encodes a guanine nucleotide exchange factor that potentially links Rho and Rac signaling pathways.	bind
54118	4	11456	6	10	NULL	0	NULL	ost			is a type of					oncogene					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_9_4986_s_376	9710582	A novel oncogene, ost, encodes a guanine nucleotide exchange factor that potentially links Rho and Rac signaling pathways.	bind
50936	1	11462	5	NULL	NULL	NULL	NULL	Siah	GP	mammalian	is a homolog of					Sina	GP	Drosophila			NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_5_915_s_3	11389839	A novel pathway for  -catenin degradation was discovered involving mammalian homologs of  Drosophila Sina (Siah), which bind ubiquitin-conjugating enzymes, and Ebi, an F box protein that binds  -catenin independent of the phosphorylation sites recognized by  -TrCP.	bind
50937	2	11462	5	NULL	NULL	NULL	NULL	Siah	GP	mammalian	bind					ubiquitin-conjugating enzymes	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_5_915_s_3	11389839	A novel pathway for  -catenin degradation was discovered involving mammalian homologs of  Drosophila Sina (Siah), which bind ubiquitin-conjugating enzymes, and Ebi, an F box protein that binds  -catenin independent of the phosphorylation sites recognized by  -TrCP.	bind
50938	3	11462	5	NULL	NULL	NULL	NULL	Siah	GP	mammalian	bind					Ebi	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_5_915_s_3	11389839	A novel pathway for  -catenin degradation was discovered involving mammalian homologs of  Drosophila Sina (Siah), which bind ubiquitin-conjugating enzymes, and Ebi, an F box protein that binds  -catenin independent of the phosphorylation sites recognized by  -TrCP.	bind
50939	4	11462	5	NULL	NULL	NULL	NULL	Ebi	GP		is a type of					F box protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_5_915_s_3	11389839	A novel pathway for  -catenin degradation was discovered involving mammalian homologs of  Drosophila Sina (Siah), which bind ubiquitin-conjugating enzymes, and Ebi, an F box protein that binds  -catenin independent of the phosphorylation sites recognized by  -TrCP.	bind
50940	5	11462	5	NULL	NULL	NULL	NULL	Ebi	GP		bind					catenin	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_5_915_s_3	11389839	A novel pathway for  -catenin degradation was discovered involving mammalian homologs of  Drosophila Sina (Siah), which bind ubiquitin-conjugating enzymes, and Ebi, an F box protein that binds  -catenin independent of the phosphorylation sites recognized by  -TrCP.	bind
50941	6	11462	5	NULL	NULL	NULL	NULL	TrCP	GP		recognizes					phosphorylation sites	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_5_915_s_3	11389839	A novel pathway for  -catenin degradation was discovered involving mammalian homologs of  Drosophila Sina (Siah), which bind ubiquitin-conjugating enzymes, and Ebi, an F box protein that binds  -catenin independent of the phosphorylation sites recognized by  -TrCP.	bind
50942	7	11462	5	NULL	NULL	NULL	NULL	statement 5	Process		is independent of					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_5_915_s_3	11389839	A novel pathway for  -catenin degradation was discovered involving mammalian homologs of  Drosophila Sina (Siah), which bind ubiquitin-conjugating enzymes, and Ebi, an F box protein that binds  -catenin independent of the phosphorylation sites recognized by  -TrCP.	bind
47862	1	11462	6	10	NULL	0	NULL	Siah		mammalian	is a homolog of					Sina		Drosophila			NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_5_915_s_3	11389839	A novel pathway for  -catenin degradation was discovered involving mammalian homologs of  Drosophila Sina (Siah), which bind ubiquitin-conjugating enzymes, and Ebi, an F box protein that binds  -catenin independent of the phosphorylation sites recognized by  -TrCP.	bind
47863	2	11462	6	10	NULL	0	NULL	Siah		mammalian	bind					ubiquitin-conjugating enzyme					NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_5_915_s_3	11389839	A novel pathway for  -catenin degradation was discovered involving mammalian homologs of  Drosophila Sina (Siah), which bind ubiquitin-conjugating enzymes, and Ebi, an F box protein that binds  -catenin independent of the phosphorylation sites recognized by  -TrCP.	bind
47864	3	11462	6	10	NULL	0	NULL	Siah		 mammalian	bind					Ebi					NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_5_915_s_3	11389839	A novel pathway for  -catenin degradation was discovered involving mammalian homologs of  Drosophila Sina (Siah), which bind ubiquitin-conjugating enzymes, and Ebi, an F box protein that binds  -catenin independent of the phosphorylation sites recognized by  -TrCP.	bind
47865	4	11462	6	10	NULL	0	NULL	Ebi			bind					catenin					NULL		NULL	NULL	NULL	NULL	gw60_molcell_7_5_915_s_3	11389839	A novel pathway for  -catenin degradation was discovered involving mammalian homologs of  Drosophila Sina (Siah), which bind ubiquitin-conjugating enzymes, and Ebi, an F box protein that binds  -catenin independent of the phosphorylation sites recognized by  -TrCP.	bind
47866	5	11462	6	NULL	NULL	0	NULL		NULL		are recognized by	NULL		phosphorylation sites		TrCP	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_7_5_915_s_3	11389839	A novel pathway for  -catenin degradation was discovered involving mammalian homologs of  Drosophila Sina (Siah), which bind ubiquitin-conjugating enzymes, and Ebi, an F box protein that binds  -catenin independent of the phosphorylation sites recognized by  -TrCP.	bind
47867	6	11462	6	NULL	NULL	0	NULL	statement 4	NULL		is independent of	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_7_5_915_s_3	11389839	A novel pathway for  -catenin degradation was discovered involving mammalian homologs of  Drosophila Sina (Siah), which bind ubiquitin-conjugating enzymes, and Ebi, an F box protein that binds  -catenin independent of the phosphorylation sites recognized by  -TrCP.	bind
54119	7	11462	6	10	NULL	0	NULL	Ebi			is a type of					F box protein					NULL		0	NULL	NULL	NULL	gw60_molcell_7_5_915_s_3	11389839	A novel pathway for  -catenin degradation was discovered involving mammalian homologs of  Drosophila Sina (Siah), which bind ubiquitin-conjugating enzymes, and Ebi, an F box protein that binds  -catenin independent of the phosphorylation sites recognized by  -TrCP.	bind
50943	1	11464	5	NULL	NULL	NULL	NULL	ESX1	GP		is a type of					homeoprotein	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_9_2376_s_337	9171351	A Novel PF/PN Motif Inhibits Nuclear Localization and DNA Binding Activity of the ESX1 Homeoprotein.	bind
50944	2	11464	5	NULL	NULL	NULL	NULL	ESX1	GP		is localized to					nucleus	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_9_2376_s_337	9171351	A Novel PF/PN Motif Inhibits Nuclear Localization and DNA Binding Activity of the ESX1 Homeoprotein.	bind
50945	3	11464	5	NULL	NULL	NULL	NULL				inhibit			PF/PN motif		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_9_2376_s_337	9171351	A Novel PF/PN Motif Inhibits Nuclear Localization and DNA Binding Activity of the ESX1 Homeoprotein.	bind
50946	4	11464	5	NULL	NULL	NULL	NULL	ESX1	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_9_2376_s_337	9171351	A Novel PF/PN Motif Inhibits Nuclear Localization and DNA Binding Activity of the ESX1 Homeoprotein.	bind
50947	5	11464	5	NULL	NULL	NULL	NULL				inhibit			PF/PN motif		statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_9_2376_s_337	9171351	A Novel PF/PN Motif Inhibits Nuclear Localization and DNA Binding Activity of the ESX1 Homeoprotein.	bind
47708	1	11464	6	10	NULL	0	NULL	ESX1 			bind					DNA					NULL		NULL	NULL	NULL	NULL	gw60_embo_16_9_2376_s_337	9171351	A Novel PF/PN Motif Inhibits Nuclear Localization and DNA Binding Activity of the ESX1 Homeoprotein.	bind
47709	2	11464	6	10	NULL	0	NULL	ESX1			localizes to					nucleus					NULL		NULL	NULL	NULL	NULL	gw60_embo_16_9_2376_s_337	9171351	A Novel PF/PN Motif Inhibits Nuclear Localization and DNA Binding Activity of the ESX1 Homeoprotein.	bind
47710	3	11464	6	NULL	NULL	0	NULL		NULL		inhibits	NULL		PF/PN Motif		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_16_9_2376_s_337	9171351	A Novel PF/PN Motif Inhibits Nuclear Localization and DNA Binding Activity of the ESX1 Homeoprotein.	bind
47711	4	11464	6	NULL	NULL	0	NULL		NULL		inhibits	NULL		PF/PN Motif		statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_16_9_2376_s_337	9171351	A Novel PF/PN Motif Inhibits Nuclear Localization and DNA Binding Activity of the ESX1 Homeoprotein.	bind
54121	5	11464	6	10	NULL	0	NULL	ESX1			is a type of					homeoprotein					NULL		0	NULL	NULL	NULL	gw60_embo_16_9_2376_s_337	9171351	A Novel PF/PN Motif Inhibits Nuclear Localization and DNA Binding Activity of the ESX1 Homeoprotein.	bind
50948	1	11465	5	NULL	NULL	NULL	NULL	hINV gene	GP	activation of;;expression of	is dependent on					phorbol ester	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_19_17032_s_24	11864971	A novel PKC, Ras, MEKK1, MEK3/MEK6, p38 pathway has been shown to mediate phorbol ester-dependent activation of  hINV gene expression ( 28-30).	bind
50949	2	11465	5	NULL	NULL	NULL	NULL	PKC pathway	Process	novel	mediate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_19_17032_s_24	11864971	A novel PKC, Ras, MEKK1, MEK3/MEK6, p38 pathway has been shown to mediate phorbol ester-dependent activation of  hINV gene expression ( 28-30).	bind
50950	3	11465	5	NULL	NULL	NULL	NULL	Ras pathway	Process	novel	mediate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_19_17032_s_24	11864971	A novel PKC, Ras, MEKK1, MEK3/MEK6, p38 pathway has been shown to mediate phorbol ester-dependent activation of  hINV gene expression ( 28-30).	bind
50951	4	11465	5	NULL	NULL	NULL	NULL	MEKK1 pathway	Process	novel	mediate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_19_17032_s_24	11864971	A novel PKC, Ras, MEKK1, MEK3/MEK6, p38 pathway has been shown to mediate phorbol ester-dependent activation of  hINV gene expression ( 28-30).	bind
50952	5	11465	5	NULL	NULL	NULL	NULL	MEK3/MEK6 pathway	Process	novel	mediate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_19_17032_s_24	11864971	A novel PKC, Ras, MEKK1, MEK3/MEK6, p38 pathway has been shown to mediate phorbol ester-dependent activation of  hINV gene expression ( 28-30).	bind
50953	6	11465	5	NULL	NULL	NULL	NULL	p38 pathway	Process	novel	mediate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_19_17032_s_24	11864971	A novel PKC, Ras, MEKK1, MEK3/MEK6, p38 pathway has been shown to mediate phorbol ester-dependent activation of  hINV gene expression ( 28-30).	bind
47712	1	11465	6	10	NULL	0	NULL	hINV gene		activation of;;expression of	is dependent on					phorbol ester					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_19_17032_s_24	11864971	A novel PKC, Ras, MEKK1, MEK3/MEK6, p38 pathway has been shown to mediate phorbol ester-dependent activation of  hINV gene expression ( 28-30).	bind
47868	2	11465	6	NULL	NULL	0	NULL	PKC pathway	NULL	novel	mediates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_19_17032_s_24	11864971	A novel PKC, Ras, MEKK1, MEK3/MEK6, p38 pathway has been shown to mediate phorbol ester-dependent activation of  hINV gene expression ( 28-30).	bind
47869	3	11465	6	NULL	NULL	0	NULL	Ras pathway	NULL	novel	mediates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_19_17032_s_24	11864971	A novel PKC, Ras, MEKK1, MEK3/MEK6, p38 pathway has been shown to mediate phorbol ester-dependent activation of  hINV gene expression ( 28-30).	bind
47870	4	11465	6	NULL	NULL	0	NULL	MEKK1 pathway	NULL	novel	mediates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_19_17032_s_24	11864971	A novel PKC, Ras, MEKK1, MEK3/MEK6, p38 pathway has been shown to mediate phorbol ester-dependent activation of  hINV gene expression ( 28-30).	bind
47871	5	11465	6	NULL	NULL	0	NULL	MEK3/MEK6 pathway	NULL	novel	mediates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_19_17032_s_24	11864971	A novel PKC, Ras, MEKK1, MEK3/MEK6, p38 pathway has been shown to mediate phorbol ester-dependent activation of  hINV gene expression ( 28-30).	bind
47872	6	11465	6	NULL	NULL	0	NULL	p38 pathway	NULL	novel	mediates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_19_17032_s_24	11864971	A novel PKC, Ras, MEKK1, MEK3/MEK6, p38 pathway has been shown to mediate phorbol ester-dependent activation of  hINV gene expression ( 28-30).	bind
50954	1	11468	5	NULL	NULL	NULL	NULL	virus	Organism		induce					IFN-A genes	GP	transcription of			NULL		NULL	NULL	NULL	NULL	abs-batch0560-0569_nucleic-acids-res_23_24_8559665_s_1	8559665	A novel PRD I and TG binding activity involved in virus-induced transcription of IFN-A genes..	bind
50955	2	11468	5	NULL	NULL	NULL	NULL	PRD I	GP	binding activity of	involves					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0560-0569_nucleic-acids-res_23_24_8559665_s_1	8559665	A novel PRD I and TG binding activity involved in virus-induced transcription of IFN-A genes..	bind
50956	3	11468	5	NULL	NULL	NULL	NULL	TG	GP	binding activity of	involves					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0560-0569_nucleic-acids-res_23_24_8559665_s_1	8559665	A novel PRD I and TG binding activity involved in virus-induced transcription of IFN-A genes..	bind
47714	1	11468	6	NULL	NULL	0	NULL	virus	NULL		induces	NULL				IFN-A genes	NULL	transcription of			NULL		0	NULL	NULL	NULL	abs-batch0560-0569_nucleic-acids-res_23_24_8559665_s_1	8559665	A novel PRD I and TG binding activity involved in virus-induced transcription of IFN-A genes..	bind
47715	2	11468	6	NULL	NULL	0	NULL	PRD I	NULL	binding activity of	is involved in	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0560-0569_nucleic-acids-res_23_24_8559665_s_1	8559665	A novel PRD I and TG binding activity involved in virus-induced transcription of IFN-A genes..	bind
47716	3	11468	6	NULL	NULL	0	NULL	TG	NULL	binding activity of	is involved in	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0560-0569_nucleic-acids-res_23_24_8559665_s_1	8559665	A novel PRD I and TG binding activity involved in virus-induced transcription of IFN-A genes..	bind
50957	1	11469	5	NULL	NULL	NULL	NULL	RGPR-p117	GP		is a type of					regucalcin gene promoter region-related protein	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0540-0549_int-j-mol-med_16_6_16273285_s_2	16273285	A novel protein RGPR-p117 was discovered as a regucalcin gene promoter  region-related protein that binds to the TTGGC motif using a yeast one-hybrid  system.	bind
50958	2	11469	5	NULL	NULL	NULL	NULL	RGPR-p117	GP		bind									TTGGC motif	NULL		NULL	NULL	NULL	NULL	abs-batch0540-0549_int-j-mol-med_16_6_16273285_s_2	16273285	A novel protein RGPR-p117 was discovered as a regucalcin gene promoter  region-related protein that binds to the TTGGC motif using a yeast one-hybrid  system.	bind
47717	1	11469	6	NULL	NULL	0	NULL	RGPR-p117 protein	NULL		is a type of	NULL				regucalcin gene promoter region-related protein	NULL				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_int-j-mol-med_16_6_16273285_s_2	16273285	A novel protein RGPR-p117 was discovered as a regucalcin gene promoter  region-related protein that binds to the TTGGC motif using a yeast one-hybrid  system.	bind
47718	2	11469	6	NULL	NULL	0	NULL	RGPR-p117 protein	NULL		bind	NULL					NULL			TTGGC motif	NULL		0	NULL	NULL	NULL	abs-batch0540-0549_int-j-mol-med_16_6_16273285_s_2	16273285	A novel protein RGPR-p117 was discovered as a regucalcin gene promoter  region-related protein that binds to the TTGGC motif using a yeast one-hybrid  system.	bind
50959	1	11473	5	NULL	NULL	NULL	NULL	Btf	GP		is					Bcl-2-associated transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4390_s_7	10330179	A novel protein, Btf (Bcl-2-associated transcription factor), that interacts with E1B 19K as well as with the antiapoptotic family members Bcl-2 and Bcl-xL but not with the proapoptotic protein Bax was identified.	bind
50960	2	11473	5	NULL	NULL	NULL	NULL	Btf	GP		interacts with					E1B 19K	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4390_s_7	10330179	A novel protein, Btf (Bcl-2-associated transcription factor), that interacts with E1B 19K as well as with the antiapoptotic family members Bcl-2 and Bcl-xL but not with the proapoptotic protein Bax was identified.	bind
50961	3	11473	5	NULL	NULL	NULL	NULL	Bcl-2	GP		is a member of					antiapoptotic family	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4390_s_7	10330179	A novel protein, Btf (Bcl-2-associated transcription factor), that interacts with E1B 19K as well as with the antiapoptotic family members Bcl-2 and Bcl-xL but not with the proapoptotic protein Bax was identified.	bind
50962	4	11473	5	NULL	NULL	NULL	NULL	Bcl-xL	GP		is a member of					antiapoptotic family	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4390_s_7	10330179	A novel protein, Btf (Bcl-2-associated transcription factor), that interacts with E1B 19K as well as with the antiapoptotic family members Bcl-2 and Bcl-xL but not with the proapoptotic protein Bax was identified.	bind
50963	5	11473	5	NULL	NULL	NULL	NULL	Btf	GP		interacts with					Bcl-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4390_s_7	10330179	A novel protein, Btf (Bcl-2-associated transcription factor), that interacts with E1B 19K as well as with the antiapoptotic family members Bcl-2 and Bcl-xL but not with the proapoptotic protein Bax was identified.	bind
50964	6	11473	5	NULL	NULL	NULL	NULL	Btf	GP		interacts with					Bcl-xL	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4390_s_7	10330179	A novel protein, Btf (Bcl-2-associated transcription factor), that interacts with E1B 19K as well as with the antiapoptotic family members Bcl-2 and Bcl-xL but not with the proapoptotic protein Bax was identified.	bind
50965	7	11473	5	NULL	NULL	NULL	NULL	Bax	GP		is a type of					proapoptotic protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4390_s_7	10330179	A novel protein, Btf (Bcl-2-associated transcription factor), that interacts with E1B 19K as well as with the antiapoptotic family members Bcl-2 and Bcl-xL but not with the proapoptotic protein Bax was identified.	bind
50966	8	11473	5	NULL	NULL	NULL	NULL	Btf	GP		does not interact with					Bax	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4390_s_7	10330179	A novel protein, Btf (Bcl-2-associated transcription factor), that interacts with E1B 19K as well as with the antiapoptotic family members Bcl-2 and Bcl-xL but not with the proapoptotic protein Bax was identified.	bind
47719	1	11473	6	NULL	NULL	0	NULL	Btf	NULL		is	NULL				Bcl-2-associated transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_6_4390_s_7	10330179	A novel protein, Btf (Bcl-2-associated transcription factor), that interacts with E1B 19K as well as with the antiapoptotic family members Bcl-2 and Bcl-xL but not with the proapoptotic protein Bax was identified.	bind
47720	2	11473	6	10	NULL	0	NULL	Btf			interacts with					E1B 19K					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4390_s_7	10330179	A novel protein, Btf (Bcl-2-associated transcription factor), that interacts with E1B 19K as well as with the antiapoptotic family members Bcl-2 and Bcl-xL but not with the proapoptotic protein Bax was identified.	bind
47721	3	11473	6	10	NULL	0	NULL	Btf			interacts with					Bcl-2					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4390_s_7	10330179	A novel protein, Btf (Bcl-2-associated transcription factor), that interacts with E1B 19K as well as with the antiapoptotic family members Bcl-2 and Bcl-xL but not with the proapoptotic protein Bax was identified.	bind
47722	4	11473	6	10	NULL	0	NULL	Btf			interacts with					Bcl-xL					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4390_s_7	10330179	A novel protein, Btf (Bcl-2-associated transcription factor), that interacts with E1B 19K as well as with the antiapoptotic family members Bcl-2 and Bcl-xL but not with the proapoptotic protein Bax was identified.	bind
47723	5	11473	6	NULL	NULL	0	NULL	Bcl-2	NULL		is a type of	NULL				antiapoptotic family member	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_6_4390_s_7	10330179	A novel protein, Btf (Bcl-2-associated transcription factor), that interacts with E1B 19K as well as with the antiapoptotic family members Bcl-2 and Bcl-xL but not with the proapoptotic protein Bax was identified.	bind
47724	6	11473	6	NULL	NULL	0	NULL	Bcl-xL	NULL		is a type of	NULL				antiapoptotic family member	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_6_4390_s_7	10330179	A novel protein, Btf (Bcl-2-associated transcription factor), that interacts with E1B 19K as well as with the antiapoptotic family members Bcl-2 and Bcl-xL but not with the proapoptotic protein Bax was identified.	bind
47725	7	11473	6	10	NULL	0	NULL	Btf			does not interact with					Bax					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4390_s_7	10330179	A novel protein, Btf (Bcl-2-associated transcription factor), that interacts with E1B 19K as well as with the antiapoptotic family members Bcl-2 and Bcl-xL but not with the proapoptotic protein Bax was identified.	bind
47726	8	11473	6	NULL	NULL	0	NULL	Bax	NULL		is a type of	NULL				proapoptotic protein	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_6_4390_s_7	10330179	A novel protein, Btf (Bcl-2-associated transcription factor), that interacts with E1B 19K as well as with the antiapoptotic family members Bcl-2 and Bcl-xL but not with the proapoptotic protein Bax was identified.	bind
50967	2	11474	5	NULL	NULL	NULL	NULL	chimeric T-cell receptors	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_clinmicrobiolrev_11_1_42_s_221	9457428	A novel protocol recently begun involves the redirection of the antigenic specificity of CD8-cell populations through the introduction of genes encoding chimeric T-cell receptors that bind HIV-1-infected cells.	bind
50968	1	11474	5	NULL	NULL	NULL	NULL	cells	Cell		infected by					HIV-1	Organism				NULL		NULL	NULL	NULL	NULL	gw60_clinmicrobiolrev_11_1_42_s_221	9457428	A novel protocol recently begun involves the redirection of the antigenic specificity of CD8-cell populations through the introduction of genes encoding chimeric T-cell receptors that bind HIV-1-infected cells.	bind
47727	2	11474	6	10	NULL	0	NULL	chimeric T-cell receptors			bind					HIV-1 infected cells					NULL		NULL	NULL	NULL	NULL	gw60_clinmicrobiolrev_11_1_42_s_221	9457428	A novel protocol recently begun involves the redirection of the antigenic specificity of CD8-cell populations through the introduction of genes encoding chimeric T-cell receptors that bind HIV-1-infected cells.	bind
58569	1	11474	6	10	NULL	0	NULL	cells			infected by					HIV					NULL		0	NULL	NULL	NULL	gw60_clinmicrobiolrev_11_1_42_s_221	9457428	A novel protocol recently begun involves the redirection of the antigenic specificity of CD8-cell populations through the introduction of genes encoding chimeric T-cell receptors that bind HIV-1-infected cells.	bind
50969	1	11475	5	NULL	NULL	NULL	NULL	MYT2	GP		is a type of					putative transcription factor protein	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_febs-lett_473_3_10818241_s_1	10818241	A novel putative transcription factor protein MYT2 that preferentially binds supercoiled DNA and induces DNA synthesis in quiescent cells..	bind
50970	2	11475	5	NULL	NULL	NULL	NULL	MYT2	GP		bind		preferentially			supercoiled DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_febs-lett_473_3_10818241_s_1	10818241	A novel putative transcription factor protein MYT2 that preferentially binds supercoiled DNA and induces DNA synthesis in quiescent cells..	bind
50971	3	11475	5	NULL	NULL	NULL	NULL	MYT2	GP		induce					DNA	NucleicAcid	synthesis of			NULL	quiescent cells	NULL	NULL	NULL	NULL	abs-batch0720-0739_febs-lett_473_3_10818241_s_1	10818241	A novel putative transcription factor protein MYT2 that preferentially binds supercoiled DNA and induces DNA synthesis in quiescent cells..	bind
47728	1	11475	6	NULL	NULL	0	NULL	MYT2 protein	NULL		is a type of	NULL				putative transcription factor	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_febs-lett_473_3_10818241_s_1	10818241	A novel putative transcription factor protein MYT2 that preferentially binds supercoiled DNA and induces DNA synthesis in quiescent cells..	bind
47729	2	11475	6	NULL	NULL	0	NULL	MYT2 protein	NULL		bind	NULL	preferentially			supercoiled DNA	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_febs-lett_473_3_10818241_s_1	10818241	A novel putative transcription factor protein MYT2 that preferentially binds supercoiled DNA and induces DNA synthesis in quiescent cells..	bind
47730	3	11475	6	NULL	NULL	0	NULL	MYT2 protein	NULL		induces	NULL				DNA	NULL	synthesis of			NULL	quiescent cells	0	NULL	NULL	NULL	abs-batch0720-0739_febs-lett_473_3_10818241_s_1	10818241	A novel putative transcription factor protein MYT2 that preferentially binds supercoiled DNA and induces DNA synthesis in quiescent cells..	bind
50972	1	11476	5	NULL	NULL	NULL	NULL	vitellogenin	GP	(DIG)-labeled	bind					ovarian membrane proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_67_2_655_s_7	12135911	A novel receptor-binding assay for vitellogenin was developed based on digoxigenin (DIG)-labeled vitellogenin tracer binding to ovarian membrane proteins immobilized in 96-well plates.	bind
47731	1	11476	6	10	NULL	0	NULL	vitellogenin tracer		(DIG)-labeled	bind					ovarian membrane proteins					NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_67_2_655_s_7	12135911	A novel receptor-binding assay for vitellogenin was developed based on digoxigenin (DIG)-labeled vitellogenin tracer binding to ovarian membrane proteins immobilized in 96-well plates.	bind
50973	1	11477	5	NULL	NULL	NULL	NULL	H+-V-ATPase	GP		bind					actin cytoskeleton	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_20_18499_s_1	12606563	A novel role for subunit C in mediating binding of the H+-V-ATPase to the actin cytoskeleton.	bind
50974	2	11477	5	NULL	NULL	NULL	NULL				mediate			subunit C		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_20_18499_s_1	12606563	A novel role for subunit C in mediating binding of the H+-V-ATPase to the actin cytoskeleton.	bind
47732	1	11477	6	NULL	NULL	0	NULL	H+-V-ATPase	NULL		bind	NULL				actin cytoskeleton	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_20_18499_s_1	12606563	A novel role for subunit C in mediating binding of the H+-V-ATPase to the actin cytoskeleton.	bind
47733	2	11477	6	NULL	NULL	0	NULL		NULL		mediates	NULL		subunit C		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_20_18499_s_1	12606563	A novel role for subunit C in mediating binding of the H+-V-ATPase to the actin cytoskeleton.	bind
50975	1	11478	5	NULL	NULL	NULL	NULL	Fen1/Rad27	GP		bind					PCNA	GP				NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_67_0_721_s_699	9759502	A Novel Role in DNA Metabolism for the Binding of Fen1/Rad27 to PCNA and Implications for Genetic Risk.	bind
50976	2	11478	5	NULL	NULL	NULL	NULL	statement 1	Process		plays a role in					DNA	NucleicAcid	metabolism of			NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_67_0_721_s_699	9759502	A Novel Role in DNA Metabolism for the Binding of Fen1/Rad27 to PCNA and Implications for Genetic Risk.	bind
47734	1	11478	6	NULL	NULL	0	NULL	Fen1/Rad27	NULL		bind	NULL				PCNA	NULL				NULL		0	NULL	NULL	NULL	gw60_annrevbiochem_67_0_721_s_699	9759502	A Novel Role in DNA Metabolism for the Binding of Fen1/Rad27 to PCNA and Implications for Genetic Risk.	bind
47735	2	11478	6	10	NULL	0	NULL	statement 1			plays a role in					DNA		metabolism of			NULL		NULL	NULL	NULL	NULL	gw60_annrevbiochem_67_0_721_s_699	9759502	A Novel Role in DNA Metabolism for the Binding of Fen1/Rad27 to PCNA and Implications for Genetic Risk.	bind
50977	1	11479	5	NULL	NULL	NULL	NULL	serine threonine kinase	GP	novel	bind					Ras-related RhoA GTPase	GP				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_3_195_s_180	10926869	A novel serine threonine kinase binding the Ras-related RhoA GTPase which translocate the kinase to peripheral membranes.	bind
50978	2	11479	5	NULL	NULL	NULL	NULL	serine threonine kinase	GP	novel	is translocated to					peripheral membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_3_195_s_180	10926869	A novel serine threonine kinase binding the Ras-related RhoA GTPase which translocate the kinase to peripheral membranes.	bind
50979	3	11479	5	NULL	NULL	NULL	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_3_195_s_180	10926869	A novel serine threonine kinase binding the Ras-related RhoA GTPase which translocate the kinase to peripheral membranes.	bind
47782	1	11479	6	NULL	NULL	0	NULL	serine threonine kinase	NULL		bind	NULL				Ras-related RhoA GTPase	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_3_195_s_180	10926869	A novel serine threonine kinase binding the Ras-related RhoA GTPase which translocate the kinase to peripheral membranes.	bind
47785	2	11479	6	10	NULL	0	NULL	serine threonine kinase			translocated to					peripheral membrane					NULL		NULL	NULL	NULL	NULL	gw60_circulationres_87_3_195_s_180	10926869	A novel serine threonine kinase binding the Ras-related RhoA GTPase which translocate the kinase to peripheral membranes.	bind
47786	3	11479	6	NULL	NULL	0	NULL	Ras-related RhoA GTPase	NULL		performs	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_87_3_195_s_180	10926869	A novel serine threonine kinase binding the Ras-related RhoA GTPase which translocate the kinase to peripheral membranes.	bind
50980	1	11490	5	NULL	NULL	NULL	NULL	shuttle protein	GP	novel	bind					RNA helicase A	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_160_2_177_s_569	12538639	A Novel Shuttle Protein Binds to RNA Helicase A and Activates the Retroviral Constitutive Transport Element.	bind
50981	2	11490	5	NULL	NULL	NULL	NULL	statement 1	Process		activates					retroviral constitutive transport element	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_160_2_177_s_569	12538639	A Novel Shuttle Protein Binds to RNA Helicase A and Activates the Retroviral Constitutive Transport Element.	bind
47787	1	11490	6	NULL	NULL	0	NULL	Shuttle Protein	NULL		bind	NULL				RNA Helicase A	NULL				NULL		0	NULL	NULL	NULL	gw60_cellbiol_160_2_177_s_569	12538639	A Novel Shuttle Protein Binds to RNA Helicase A and Activates the Retroviral Constitutive Transport Element.	bind
47788	2	11490	6	10	NULL	0	NULL	statement 1			activates					retroviral Constitutive Transport Element					NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_160_2_177_s_569	12538639	A Novel Shuttle Protein Binds to RNA Helicase A and Activates the Retroviral Constitutive Transport Element.	bind
50982	1	11491	5	NULL	NULL	NULL	NULL	EphA2	GP		is activated by					ligand	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_3_1303_s_20	9430661	A novel Src homologous adapter protein, SLAP, also binds ligand-activated EphA2 ( 14).	bind
50983	2	11491	5	NULL	NULL	NULL	NULL	SLAP	GP		bind					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_3_1303_s_20	9430661	A novel Src homologous adapter protein, SLAP, also binds ligand-activated EphA2 ( 14).	bind
50984	3	11491	5	NULL	NULL	NULL	NULL	SLAP	GP		is a type of					Src homologous adapter protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_3_1303_s_20	9430661	A novel Src homologous adapter protein, SLAP, also binds ligand-activated EphA2 ( 14).	bind
47789	2	11491	6	10	NULL	0	NULL	SLAP			bind					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_3_1303_s_20	9430661	A novel Src homologous adapter protein, SLAP, also binds ligand-activated EphA2 ( 14).	bind
47790	3	11491	6	10	NULL	0	NULL	SLAP			is a type of					Src homologous adapter protein					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_3_1303_s_20	9430661	A novel Src homologous adapter protein, SLAP, also binds ligand-activated EphA2 ( 14).	bind
54122	1	11491	6	10	NULL	0	NULL	ligand			activates					EphA2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_3_1303_s_20	9430661	A novel Src homologous adapter protein, SLAP, also binds ligand-activated EphA2 ( 14).	bind
50985	1	11492	5	NULL	NULL	NULL	NULL	GAKIN	GP		bind			stalk segment		hDlg	GP		GUK Domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_10_8395_s_110	12496241	A Novel Stalk Segment of GAKIN Binds to the GUK Domain of hDlg-- To map the hDlg-binding site within GAKIN, a series of truncated constructs of GAKIN were engineered and expressed in the rabbit reticulocyte transcription/translation system.	bind
47791	1	11492	6	NULL	NULL	0	NULL	GAKIN	NULL		bind	NULL		stalk segment		hDlg	NULL		GUK domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_10_8395_s_110	12496241	A Novel Stalk Segment of GAKIN Binds to the GUK Domain of hDlg-- To map the hDlg-binding site within GAKIN, a series of truncated constructs of GAKIN were engineered and expressed in the rabbit reticulocyte transcription/translation system.	bind
50986	1	11493	5	NULL	NULL	NULL	NULL	semaphorin	GP		is a type of					transmembrane protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_nature_410_6825_174_s_254	11242070	A novel transmembrane semaphorin can bind c-src.	bind
50987	2	11493	5	NULL	NULL	NULL	NULL	semaphorin	GP		bind					c-src	GP				NULL		NULL	NULL	NULL	NULL	gw60_nature_410_6825_174_s_254	11242070	A novel transmembrane semaphorin can bind c-src.	bind
47792	1	11493	6	10	NULL	0	NULL	semaphorin			bind					c-src					NULL		NULL	NULL	NULL	NULL	gw60_nature_410_6825_174_s_254	11242070	A novel transmembrane semaphorin can bind c-src.	bind
54123	2	11493	6	10	NULL	0	NULL	semaphorin			is a type of					transmembrane protein					NULL		0	NULL	NULL	NULL	gw60_nature_410_6825_174_s_254	11242070	A novel transmembrane semaphorin can bind c-src.	bind
50988	1	11494	5	NULL	NULL	NULL	NULL	NSD1	GP		bind								holo-LBDs		NULL		NULL	NULL	NULL	NULL	gw60_embo_17_12_3398_s_7	9628876	A novel variant (FxxLL) of the NR box motif (LxxLL) is present in NID+L and is required for the binding of NSD1 to holo-LBDs.	bind
50989	2	11494	5	10	NULL	0	NULL				is a variant of				FxxLL					NR box motif LxxLL	NULL		NULL	NULL	NULL	NULL	gw60_embo_17_12_3398_s_7	9628876	A novel variant (FxxLL) of the NR box motif (LxxLL) is present in NID+L and is required for the binding of NSD1 to holo-LBDs.	bind
50990	3	11494	5	NULL	NULL	NULL	NULL	statement 2	Process		is present in					NID+L	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_12_3398_s_7	9628876	A novel variant (FxxLL) of the NR box motif (LxxLL) is present in NID+L and is required for the binding of NSD1 to holo-LBDs.	bind
50991	4	11494	5	NULL	NULL	NULL	NULL	statement 3	Process		is required for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_12_3398_s_7	9628876	A novel variant (FxxLL) of the NR box motif (LxxLL) is present in NID+L and is required for the binding of NSD1 to holo-LBDs.	bind
47793	1	11494	6	NULL	NULL	0	NULL	NSD1	NULL		bind	NULL					NULL		holo-LBD		NULL		0	NULL	NULL	NULL	gw60_embo_17_12_3398_s_7	9628876	A novel variant (FxxLL) of the NR box motif (LxxLL) is present in NID+L and is required for the binding of NSD1 to holo-LBDs.	bind
47794	2	11494	6	NULL	NULL	0	NULL		NULL		is a variant of	NULL			FxxLL		NULL			NR box motif LxxLL	NULL		0	NULL	NULL	NULL	gw60_embo_17_12_3398_s_7	9628876	A novel variant (FxxLL) of the NR box motif (LxxLL) is present in NID+L and is required for the binding of NSD1 to holo-LBDs.	bind
47795	3	11494	6	NULL	NULL	0	NULL	statement 2	NULL		is present in	NULL				NID+L	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_17_12_3398_s_7	9628876	A novel variant (FxxLL) of the NR box motif (LxxLL) is present in NID+L and is required for the binding of NSD1 to holo-LBDs.	bind
47796	4	11494	6	NULL	NULL	0	NULL		NULL		is required for	NULL			FxxLL	statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_17_12_3398_s_7	9628876	A novel variant (FxxLL) of the NR box motif (LxxLL) is present in NID+L and is required for the binding of NSD1 to holo-LBDs.	bind
50992	1	11495	5	NULL	NULL	NULL	NULL	WD repeat protein	GP		is a component of					methylosome	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6533_s_295	12192051	A novel WD repeat protein component of the methylosome binds Sm proteins.	bind
50993	2	11495	5	NULL	NULL	NULL	NULL	statement 1	Process		bind					Sm proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6533_s_295	12192051	A novel WD repeat protein component of the methylosome binds Sm proteins.	bind
47797	1	11495	6	10	NULL	0	NULL	WD repeat protein			is a component of					methylosome					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6533_s_295	12192051	A novel WD repeat protein component of the methylosome binds Sm proteins.	bind
47798	2	11495	6	10	NULL	0	NULL	statement 1			bind					Sm proteins					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_18_6533_s_295	12192051	A novel WD repeat protein component of the methylosome binds Sm proteins.	bind
50994	1	11497	5	NULL	NULL	NULL	NULL	bZIP protein	GP	yeast	bind									CRE motif	NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_14_0_459_s_608	9891790	A novel yeast bZIP protein binding to the CRE motif is a multicopy  suppressor for  cdc10 mutant of  Schizosaccharomyces pombe.	bind
50995	2	11497	5	NULL	NULL	NULL	NULL	statement 1	Process		is a suppressor for					cdc10	GP	mutant;;Schizosaccharomyces pombe			NULL		NULL	NULL	NULL	NULL	gw70_annurevcelldevbiol_14_0_459_s_608	9891790	A novel yeast bZIP protein binding to the CRE motif is a multicopy  suppressor for  cdc10 mutant of  Schizosaccharomyces pombe.	bind
47799	1	11497	6	NULL	NULL	0	NULL	bZIP protein	NULL	yeast	bind	NULL					NULL			CRE motif	NULL		0	NULL	NULL	NULL	gw70_annurevcelldevbiol_14_0_459_s_608	9891790	A novel yeast bZIP protein binding to the CRE motif is a multicopy  suppressor for  cdc10 mutant of  Schizosaccharomyces pombe.	bind
47800	2	11497	6	NULL	NULL	0	NULL	statement 1	NULL		is a suppressor for	NULL				cdc10 	NULL	Schizosaccharomyces pombe;; mutant			NULL		0	NULL	NULL	NULL	gw70_annurevcelldevbiol_14_0_459_s_608	9891790	A novel yeast bZIP protein binding to the CRE motif is a multicopy  suppressor for  cdc10 mutant of  Schizosaccharomyces pombe.	bind
50996	1	11499	5	NULL	NULL	NULL	NULL	blastopore lip-specific gene	GP	Xenopus laevis	is induced by					activin	GP				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_77_2_95_s_472	9831640	A novel, activin-inducible, blastopore lip-specific gene of  Xenopus laevis contains a fork head DNA-binding domain.	bind
54124	2	11499	5	NULL	NULL	NULL	NULL	blastopore lip-specific gene	GP	Xenopus laevis	contains								fork head DNA-binding domain		NULL		NULL	NULL	NULL	NULL	gw60_mechdev_77_2_95_s_472	9831640	A novel, activin-inducible, blastopore lip-specific gene of  Xenopus laevis contains a fork head DNA-binding domain.	bind
47801	1	11499	6	NULL	NULL	0	NULL	blastopore lip-specific gene	NULL	Xenopus laevis	is induced by	NULL				activin	NULL				NULL		NULL	NULL	NULL	NULL	gw60_mechdev_77_2_95_s_472	9831640	A novel, activin-inducible, blastopore lip-specific gene of  Xenopus laevis contains a fork head DNA-binding domain.	bind
47802	2	11499	6	NULL	NULL	0	NULL	blastopore lip-specific gene	NULL	Xenopus laevis	contains	NULL					NULL		fork head DNA-binding domain		NULL		0	NULL	NULL	NULL	gw60_mechdev_77_2_95_s_472	9831640	A novel, activin-inducible, blastopore lip-specific gene of  Xenopus laevis contains a fork head DNA-binding domain.	bind
50997	1	11500	5	NULL	NULL	NULL	NULL	erythroid cell-specific transcription factor	GP		bind									CACC element	NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_21_2778_s_608	11069894	A novel, erythroid cell-specific transcription factor that binds to the CACC element related to the kruppel family of nuclear proteins.	bind
50998	2	11500	5	NULL	NULL	NULL	NULL				is related to				CACC element	nuclear proteins	GP		kruppel family		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_21_2778_s_608	11069894	A novel, erythroid cell-specific transcription factor that binds to the CACC element related to the kruppel family of nuclear proteins.	bind
47803	1	11500	6	NULL	NULL	0	NULL	erythroid cell-specific transcription factor	NULL		bind	NULL					NULL			CACC element	NULL		0	NULL	NULL	NULL	gw60_genesdev_14_21_2778_s_608	11069894	A novel, erythroid cell-specific transcription factor that binds to the CACC element related to the kruppel family of nuclear proteins.	bind
47804	2	11500	6	10	NULL	0	NULL				is related to				CACC element	nuclear proteins			kruppel family		NULL		NULL	NULL	NULL	NULL	gw60_genesdev_14_21_2778_s_608	11069894	A novel, erythroid cell-specific transcription factor that binds to the CACC element related to the kruppel family of nuclear proteins.	bind
51000	1	11501	5	NULL	NULL	NULL	NULL	HF-1b	GP		is a type of					tissue restricted zinc finger protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_nature_407_6801_227_s_276	11001065	A novel, tissue restricted zinc finger protein (HF-1b) binds to the cardiac regulatory element (HF-1b/MEF-2) in the rat myosin light chain-2 gene.	bind
51001	2	11501	5	NULL	NULL	NULL	NULL	HF-1b	GP		bind					myosin light chain-2 gene	GP	rat		HF-1b/MEF-2	NULL		NULL	NULL	NULL	NULL	gw60_nature_407_6801_227_s_276	11001065	A novel, tissue restricted zinc finger protein (HF-1b) binds to the cardiac regulatory element (HF-1b/MEF-2) in the rat myosin light chain-2 gene.	bind
54151	3	11501	5	NULL	NULL	NULL	NULL	HF-1b/MEF-2	GP		is a type of					cardiac regulatory element	GP				NULL		NULL	NULL	NULL	NULL	gw60_nature_407_6801_227_s_276	11001065	A novel, tissue restricted zinc finger protein (HF-1b) binds to the cardiac regulatory element (HF-1b/MEF-2) in the rat myosin light chain-2 gene.	bind
50366	1	11501	6	10	NULL	0	NULL	HF-1b			bind					myosin light chain-2 gene		rat		HF-1b/MEF-2	NULL		NULL	NULL	NULL	NULL	gw60_nature_407_6801_227_s_276	11001065	A novel, tissue restricted zinc finger protein (HF-1b) binds to the cardiac regulatory element (HF-1b/MEF-2) in the rat myosin light chain-2 gene.	bind
50367	2	11501	6	10	NULL	0	NULL	HF-1b			is a type of					tissue restricted zinc finger protein					NULL		NULL	NULL	NULL	NULL	gw60_nature_407_6801_227_s_276	11001065	A novel, tissue restricted zinc finger protein (HF-1b) binds to the cardiac regulatory element (HF-1b/MEF-2) in the rat myosin light chain-2 gene.	bind
50368	3	11501	6	NULL	NULL	0	NULL	HF-1b/MEF-2	NULL		is a type of	NULL				cardiac regulatory element	NULL				NULL		0	NULL	NULL	NULL	gw60_nature_407_6801_227_s_276	11001065	A novel, tissue restricted zinc finger protein (HF-1b) binds to the cardiac regulatory element (HF-1b/MEF-2) in the rat myosin light chain-2 gene.	bind
51002	1	11506	5	NULL	NULL	NULL	NULL	glycerol phosphate dehydrogenase gene	GP	human;;mitochondrial	bind				NRF-2 site	NRF-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1576_1_1_s_163	12031478	A NRF-2 site in the human mitochondrial glycerol phosphate dehydrogenase gene binds NRF-2 and makes a major contribution to promoter activity [ 77].	bind
51003	2	11506	5	NULL	NULL	NULL	NULL	statement 1	Process		contribute to					promoter	NucleicAcid	activity of			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1576_1_1_s_163	12031478	A NRF-2 site in the human mitochondrial glycerol phosphate dehydrogenase gene binds NRF-2 and makes a major contribution to promoter activity [ 77].	bind
50369	1	11506	6	NULL	NULL	0	NULL	glycerol phosphate dehydrogenase gene	NULL	human;; mitochondrial	bind	NULL			NRF-2 site	NRF-2	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1576_1_1_s_163	12031478	A NRF-2 site in the human mitochondrial glycerol phosphate dehydrogenase gene binds NRF-2 and makes a major contribution to promoter activity [ 77].	bind
50370	2	11506	6	NULL	NULL	0	NULL	statement 1	NULL		plays a role in	NULL				promoter	NULL	activity of 			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1576_1_1_s_163	12031478	A NRF-2 site in the human mitochondrial glycerol phosphate dehydrogenase gene binds NRF-2 and makes a major contribution to promoter activity [ 77].	bind
51004	1	11507	5	NULL	NULL	NULL	NULL	CRM1	GP		bind					STAT1	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_sci-stke_2003_195_12915721_s_8	12915721	A nuclear export signal of STAT1 appears  to be masked when dimers are bound to DNA, but it becomes accessible to  the CRM1 export carrier after dissociation from DNA. CRM1 binds STAT1  and transports the transcription factor back to the cytoplasm.	bind
51005	2	11507	5	NULL	NULL	NULL	NULL	STAT1	GP		is transported to					cytoplasm	CellComponent				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_sci-stke_2003_195_12915721_s_8	12915721	A nuclear export signal of STAT1 appears  to be masked when dimers are bound to DNA, but it becomes accessible to  the CRM1 export carrier after dissociation from DNA. CRM1 binds STAT1  and transports the transcription factor back to the cytoplasm.	bind
51006	3	11507	5	NULL	NULL	NULL	NULL	statement 1	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_sci-stke_2003_195_12915721_s_8	12915721	A nuclear export signal of STAT1 appears  to be masked when dimers are bound to DNA, but it becomes accessible to  the CRM1 export carrier after dissociation from DNA. CRM1 binds STAT1  and transports the transcription factor back to the cytoplasm.	bind
51007	4	11507	5	NULL	NULL	NULL	NULL	dimers	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_sci-stke_2003_195_12915721_s_8	12915721	A nuclear export signal of STAT1 appears  to be masked when dimers are bound to DNA, but it becomes accessible to  the CRM1 export carrier after dissociation from DNA. CRM1 binds STAT1  and transports the transcription factor back to the cytoplasm.	bind
51008	5	11507	5	NULL	NULL	NULL	NULL	statement 4	Process		masks					STAT1	GP		nuclear export signal		NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_sci-stke_2003_195_12915721_s_8	12915721	A nuclear export signal of STAT1 appears  to be masked when dimers are bound to DNA, but it becomes accessible to  the CRM1 export carrier after dissociation from DNA. CRM1 binds STAT1  and transports the transcription factor back to the cytoplasm.	bind
51009	6	11507	5	NULL	NULL	NULL	NULL	STAT1	GP		is accessible to			nuclear export signal		CRM1 export carrier	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_sci-stke_2003_195_12915721_s_8	12915721	A nuclear export signal of STAT1 appears  to be masked when dimers are bound to DNA, but it becomes accessible to  the CRM1 export carrier after dissociation from DNA. CRM1 binds STAT1  and transports the transcription factor back to the cytoplasm.	bind
51010	7	11507	5	NULL	NULL	NULL	NULL	dimers	GP		dissociates from					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_sci-stke_2003_195_12915721_s_8	12915721	A nuclear export signal of STAT1 appears  to be masked when dimers are bound to DNA, but it becomes accessible to  the CRM1 export carrier after dissociation from DNA. CRM1 binds STAT1  and transports the transcription factor back to the cytoplasm.	bind
51011	8	11507	5	NULL	NULL	NULL	NULL	statement 6	Process		occurs after					statement 7	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_sci-stke_2003_195_12915721_s_8	12915721	A nuclear export signal of STAT1 appears  to be masked when dimers are bound to DNA, but it becomes accessible to  the CRM1 export carrier after dissociation from DNA. CRM1 binds STAT1  and transports the transcription factor back to the cytoplasm.	bind
50503	1	11507	6	NULL	NULL	0	NULL	CRM1	NULL		bind	NULL				STAT1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_sci-stke_2003_195_12915721_s_8	12915721	A nuclear export signal of STAT1 appears  to be masked when dimers are bound to DNA, but it becomes accessible to  the CRM1 export carrier after dissociation from DNA. CRM1 binds STAT1  and transports the transcription factor back to the cytoplasm.	bind
50504	2	11507	6	NULL	NULL	0	NULL	STAT1	NULL		is transported to	NULL				cytoplasm	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_sci-stke_2003_195_12915721_s_8	12915721	A nuclear export signal of STAT1 appears  to be masked when dimers are bound to DNA, but it becomes accessible to  the CRM1 export carrier after dissociation from DNA. CRM1 binds STAT1  and transports the transcription factor back to the cytoplasm.	bind
50505	3	11507	6	10	NULL	0	NULL	statement 1			leads to					statement 2					NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_sci-stke_2003_195_12915721_s_8	12915721	A nuclear export signal of STAT1 appears  to be masked when dimers are bound to DNA, but it becomes accessible to  the CRM1 export carrier after dissociation from DNA. CRM1 binds STAT1  and transports the transcription factor back to the cytoplasm.	bind
50506	4	11507	6	NULL	NULL	0	NULL	dimers	NULL		bind	NULL				DNA	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_sci-stke_2003_195_12915721_s_8	12915721	A nuclear export signal of STAT1 appears  to be masked when dimers are bound to DNA, but it becomes accessible to  the CRM1 export carrier after dissociation from DNA. CRM1 binds STAT1  and transports the transcription factor back to the cytoplasm.	bind
50507	5	11507	6	10	NULL	0	NULL	statement 4			masks					STAT1			nuclear export signal		NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_sci-stke_2003_195_12915721_s_8	12915721	A nuclear export signal of STAT1 appears  to be masked when dimers are bound to DNA, but it becomes accessible to  the CRM1 export carrier after dissociation from DNA. CRM1 binds STAT1  and transports the transcription factor back to the cytoplasm.	bind
50508	7	11507	6	10	NULL	0	NULL	Dimers			dissociate from					DNA					NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_sci-stke_2003_195_12915721_s_8	12915721	A nuclear export signal of STAT1 appears  to be masked when dimers are bound to DNA, but it becomes accessible to  the CRM1 export carrier after dissociation from DNA. CRM1 binds STAT1  and transports the transcription factor back to the cytoplasm.	bind
50509	6	11507	6	10	NULL	0	NULL	STAT1			is accessible to			nuclear export signal		CRM1 export carrier					NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_sci-stke_2003_195_12915721_s_8	12915721	A nuclear export signal of STAT1 appears  to be masked when dimers are bound to DNA, but it becomes accessible to  the CRM1 export carrier after dissociation from DNA. CRM1 binds STAT1  and transports the transcription factor back to the cytoplasm.	bind
50510	8	11507	6	10	NULL	0	NULL	statement 6			occurs after					statement 7					NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_sci-stke_2003_195_12915721_s_8	12915721	A nuclear export signal of STAT1 appears  to be masked when dimers are bound to DNA, but it becomes accessible to  the CRM1 export carrier after dissociation from DNA. CRM1 binds STAT1  and transports the transcription factor back to the cytoplasm.	bind
51012	1	11508	5	NULL	NULL	NULL	NULL	nuclear factor	GP		is present in		exclusively			lens cells	Cell				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_development_113_2_1782865_s_5	1782865	A nuclear factor present exclusively in lens cells binds to  the 84 bp element in the region between positions -165 and -140.	bind
51013	2	11508	5	NULL	NULL	0	NULL		NULL		is present in between	NULL			84 bp element		NULL			positions -165 and -140	NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_development_113_2_1782865_s_5	1782865	A nuclear factor present exclusively in lens cells binds to  the 84 bp element in the region between positions -165 and -140.	bind
51014	3	11508	5	NULL	NULL	NULL	NULL	statement 1	Process		bind					statement 2	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_development_113_2_1782865_s_5	1782865	A nuclear factor present exclusively in lens cells binds to  the 84 bp element in the region between positions -165 and -140.	bind
50371	1	11508	6	NULL	NULL	0	NULL	nuclear factor	NULL		is present in	NULL	exclusively			lens cells	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_development_113_2_1782865_s_5	1782865	A nuclear factor present exclusively in lens cells binds to  the 84 bp element in the region between positions -165 and -140.	bind
50372	3	11508	6	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_development_113_2_1782865_s_5	1782865	A nuclear factor present exclusively in lens cells binds to  the 84 bp element in the region between positions -165 and -140.	bind
50373	2	11508	6	NULL	NULL	0	NULL		NULL		lies in the region between	NULL			84 bp element		NULL			positions -165 and -140	NULL		0	NULL	NULL	NULL	abs-batch0650-0679_development_113_2_1782865_s_5	1782865	A nuclear factor present exclusively in lens cells binds to  the 84 bp element in the region between positions -165 and -140.	bind
51015	1	11509	5	NULL	NULL	NULL	NULL	nuclear protein	GP		bind		selectively							dyad Gpal element	NULL		NULL	NULL	NULL	NULL	gw60_genetics_157_2_699_s_205	11156990	A nuclear protein binds selectively to the dyad Gpal element:   Nuclear extracts from Drosophila embryos or specific tissues were isolated and probed with a radiolabeled double-stranded 30-bp oligonucleotide (dPalGld) corresponding to the dyad Gpal (dGpal) and flanking sequences.	bind
51016	2	11509	5	NULL	NULL	NULL	NULL	dyad Gpal	GP		is					dGpal	GP				NULL		NULL	NULL	NULL	NULL	gw60_genetics_157_2_699_s_205	11156990	A nuclear protein binds selectively to the dyad Gpal element:   Nuclear extracts from Drosophila embryos or specific tissues were isolated and probed with a radiolabeled double-stranded 30-bp oligonucleotide (dPalGld) corresponding to the dyad Gpal (dGpal) and flanking sequences.	bind
50382	1	11509	6	NULL	NULL	0	NULL	nuclear protein	NULL		bind	NULL	selectively				NULL			dyad Gpal element	NULL		NULL	NULL	NULL	NULL	gw60_genetics_157_2_699_s_205	11156990	A nuclear protein binds selectively to the dyad Gpal element:   Nuclear extracts from Drosophila embryos or specific tissues were isolated and probed with a radiolabeled double-stranded 30-bp oligonucleotide (dPalGld) corresponding to the dyad Gpal (dGpal) and flanking sequences.	bind
50383	2	11509	6	NULL	NULL	0	NULL	dyad Gpal	NULL		is	NULL				dGpal	NULL				NULL		0	NULL	NULL	NULL	gw60_genetics_157_2_699_s_205	11156990	A nuclear protein binds selectively to the dyad Gpal element:   Nuclear extracts from Drosophila embryos or specific tissues were isolated and probed with a radiolabeled double-stranded 30-bp oligonucleotide (dPalGld) corresponding to the dyad Gpal (dGpal) and flanking sequences.	bind
51017	1	11510	5	NULL	NULL	NULL	NULL	nuclear protein	GP		bind		specifically							A CGTG intrinsic DNA bending sequence	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_3_1282_s_102	7836392	A Nuclear Protein Binds Specifically to the  A CGTG Intrinsic DNA Bending Sequence In preliminary  experiments we demonstrated that a protein in nuclear extracts from  CHO, HeLa, and MCF7 cells, but absent in COS cell extracts, bound  specifically to A CGTG multimers (data not shown).	bind
51018	2	11510	5	NULL	NULL	NULL	NULL	nuclear protein	GP		is present in					CHO cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_3_1282_s_102	7836392	A Nuclear Protein Binds Specifically to the  A CGTG Intrinsic DNA Bending Sequence In preliminary  experiments we demonstrated that a protein in nuclear extracts from  CHO, HeLa, and MCF7 cells, but absent in COS cell extracts, bound  specifically to A CGTG multimers (data not shown).	bind
51019	3	11510	5	NULL	NULL	NULL	NULL	nuclear protein	GP		is present in					HeLa cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_3_1282_s_102	7836392	A Nuclear Protein Binds Specifically to the  A CGTG Intrinsic DNA Bending Sequence In preliminary  experiments we demonstrated that a protein in nuclear extracts from  CHO, HeLa, and MCF7 cells, but absent in COS cell extracts, bound  specifically to A CGTG multimers (data not shown).	bind
51020	4	11510	5	NULL	NULL	NULL	NULL	nuclear protein	GP		is present in					MCF7 cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_3_1282_s_102	7836392	A Nuclear Protein Binds Specifically to the  A CGTG Intrinsic DNA Bending Sequence In preliminary  experiments we demonstrated that a protein in nuclear extracts from  CHO, HeLa, and MCF7 cells, but absent in COS cell extracts, bound  specifically to A CGTG multimers (data not shown).	bind
51021	5	11510	5	NULL	NULL	NULL	NULL	nuclear protein	GP		is absent in					COS cell extracts	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_3_1282_s_102	7836392	A Nuclear Protein Binds Specifically to the  A CGTG Intrinsic DNA Bending Sequence In preliminary  experiments we demonstrated that a protein in nuclear extracts from  CHO, HeLa, and MCF7 cells, but absent in COS cell extracts, bound  specifically to A CGTG multimers (data not shown).	bind
51022	6	11510	5	NULL	NULL	NULL	NULL	statement 2	Process		bind		specifically							A CGTG multimers	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_3_1282_s_102	7836392	A Nuclear Protein Binds Specifically to the  A CGTG Intrinsic DNA Bending Sequence In preliminary  experiments we demonstrated that a protein in nuclear extracts from  CHO, HeLa, and MCF7 cells, but absent in COS cell extracts, bound  specifically to A CGTG multimers (data not shown).	bind
54152	7	11510	5	NULL	NULL	NULL	NULL	statement 3	Process		bind		specifically							A CGTG multimers 	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_3_1282_s_102	7836392	A Nuclear Protein Binds Specifically to the  A CGTG Intrinsic DNA Bending Sequence In preliminary  experiments we demonstrated that a protein in nuclear extracts from  CHO, HeLa, and MCF7 cells, but absent in COS cell extracts, bound  specifically to A CGTG multimers (data not shown).	bind
54153	8	11510	5	NULL	NULL	NULL	NULL	statement 4	Process		bind		specifically							A CGTG multimers 	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_3_1282_s_102	7836392	A Nuclear Protein Binds Specifically to the  A CGTG Intrinsic DNA Bending Sequence In preliminary  experiments we demonstrated that a protein in nuclear extracts from  CHO, HeLa, and MCF7 cells, but absent in COS cell extracts, bound  specifically to A CGTG multimers (data not shown).	bind
50384	1	11510	6	NULL	NULL	0	NULL	nuclear protein	NULL		bind	NULL					NULL			A CGTG Intrinsic DNA Bending Sequence	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_3_1282_s_102	7836392	A Nuclear Protein Binds Specifically to the  A CGTG Intrinsic DNA Bending Sequence In preliminary  experiments we demonstrated that a protein in nuclear extracts from  CHO, HeLa, and MCF7 cells, but absent in COS cell extracts, bound  specifically to A CGTG multimers (data not shown).	bind
50385	2	11510	6	NULL	NULL	0	NULL	nuclear protein	NULL		is present in	NULL				CHO cells extracts	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_3_1282_s_102	7836392	A Nuclear Protein Binds Specifically to the  A CGTG Intrinsic DNA Bending Sequence In preliminary  experiments we demonstrated that a protein in nuclear extracts from  CHO, HeLa, and MCF7 cells, but absent in COS cell extracts, bound  specifically to A CGTG multimers (data not shown).	bind
50511	3	11510	6	NULL	NULL	0	NULL	statement 2	NULL		bind	NULL	specifically				NULL			A CGTG multimers	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_3_1282_s_102	7836392	A Nuclear Protein Binds Specifically to the  A CGTG Intrinsic DNA Bending Sequence In preliminary  experiments we demonstrated that a protein in nuclear extracts from  CHO, HeLa, and MCF7 cells, but absent in COS cell extracts, bound  specifically to A CGTG multimers (data not shown).	bind
50512	4	11510	6	NULL	NULL	0	NULL	nuclear protein	NULL		is present in	NULL				HeLa cells extracts	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_3_1282_s_102	7836392	A Nuclear Protein Binds Specifically to the  A CGTG Intrinsic DNA Bending Sequence In preliminary  experiments we demonstrated that a protein in nuclear extracts from  CHO, HeLa, and MCF7 cells, but absent in COS cell extracts, bound  specifically to A CGTG multimers (data not shown).	bind
50513	5	11510	6	NULL	NULL	0	NULL	statement 4	NULL		bind	NULL	specifically				NULL			A CGTG multimers	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_3_1282_s_102	7836392	A Nuclear Protein Binds Specifically to the  A CGTG Intrinsic DNA Bending Sequence In preliminary  experiments we demonstrated that a protein in nuclear extracts from  CHO, HeLa, and MCF7 cells, but absent in COS cell extracts, bound  specifically to A CGTG multimers (data not shown).	bind
50514	6	11510	6	NULL	NULL	0	NULL	nuclear protein	NULL		is present in	NULL				MCF7 cells extract	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_3_1282_s_102	7836392	A Nuclear Protein Binds Specifically to the  A CGTG Intrinsic DNA Bending Sequence In preliminary  experiments we demonstrated that a protein in nuclear extracts from  CHO, HeLa, and MCF7 cells, but absent in COS cell extracts, bound  specifically to A CGTG multimers (data not shown).	bind
50515	7	11510	6	10	NULL	0	NULL	statement 6			bind		specifically							A CGTG multimers	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_3_1282_s_102	7836392	A Nuclear Protein Binds Specifically to the  A CGTG Intrinsic DNA Bending Sequence In preliminary  experiments we demonstrated that a protein in nuclear extracts from  CHO, HeLa, and MCF7 cells, but absent in COS cell extracts, bound  specifically to A CGTG multimers (data not shown).	bind
54154	8	11510	6	10	NULL	0	NULL	nuclear protein			is absent in					COS cell extracts					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_3_1282_s_102	7836392	A Nuclear Protein Binds Specifically to the  A CGTG Intrinsic DNA Bending Sequence In preliminary  experiments we demonstrated that a protein in nuclear extracts from  CHO, HeLa, and MCF7 cells, but absent in COS cell extracts, bound  specifically to A CGTG multimers (data not shown).	bind
51023	1	11511	5	NULL	NULL	NULL	NULL	ZBRK1	GP		complex with					BRCA1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_4_757_s_180	11090615	A Nuclear Protein Complex Including ZBRK1 and BRCA1 Binds to the ZBRK1 Recognition Sequence in  GADD45 Intron 3	bind
51024	2	11511	5	NULL	NULL	NULL	NULL				is present in				ZBRK1 Recognition Sequence	GADD45	GP			Intron 3	NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_4_757_s_180	11090615	A Nuclear Protein Complex Including ZBRK1 and BRCA1 Binds to the ZBRK1 Recognition Sequence in  GADD45 Intron 3	bind
51025	3	11511	5	NULL	NULL	NULL	NULL	statement 1	Process		bind					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_4_757_s_180	11090615	A Nuclear Protein Complex Including ZBRK1 and BRCA1 Binds to the ZBRK1 Recognition Sequence in  GADD45 Intron 3	bind
54156	4	11511	5	NULL	NULL	NULL	NULL	statement 1	GP		is a type of					Nuclear Protein Complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_4_757_s_180	11090615	A Nuclear Protein Complex Including ZBRK1 and BRCA1 Binds to the ZBRK1 Recognition Sequence in  GADD45 Intron 3	bind
50386	1	11511	6	NULL	NULL	0	NULL	ZBRK1	NULL		forms a complex with	NULL				BRCA1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcell_6_4_757_s_180	11090615	A Nuclear Protein Complex Including ZBRK1 and BRCA1 Binds to the ZBRK1 Recognition Sequence in  GADD45 Intron 3	bind
50387	2	11511	6	10	NULL	0	NULL				present in				ZBRK1 recognition sequence	GADD45				Intron 3	NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_4_757_s_180	11090615	A Nuclear Protein Complex Including ZBRK1 and BRCA1 Binds to the ZBRK1 Recognition Sequence in  GADD45 Intron 3	bind
54155	3	11511	6	10	NULL	0	NULL	statement 1			bind					statement 2					NULL		0	NULL	NULL	NULL	gw60_molcell_6_4_757_s_180	11090615	A Nuclear Protein Complex Including ZBRK1 and BRCA1 Binds to the ZBRK1 Recognition Sequence in  GADD45 Intron 3	bind
54157	4	11511	6	10	NULL	0	NULL	statement 1			is a type of					Nuclear Protein Complex					NULL		0	NULL	NULL	NULL	gw60_molcell_6_4_757_s_180	11090615	A Nuclear Protein Complex Including ZBRK1 and BRCA1 Binds to the ZBRK1 Recognition Sequence in  GADD45 Intron 3	bind
51026	1	11512	5	NULL	NULL	NULL	NULL	nuclear protein	GP	rat;;gastric corpus	bind		specifically					putative		AP2/SP1 site	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7661_s_159	11113118	A nuclear protein isolated from rat gastric corpus also specifically bound to the putative AP2/SP1 site, as shown in Fig.  6 e.	bind
50388	1	11512	6	NULL	NULL	0	NULL	nuclear protein	NULL		is isolated from	NULL				gastric corpus	NULL	rat			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_10_7661_s_159	11113118	A nuclear protein isolated from rat gastric corpus also specifically bound to the putative AP2/SP1 site, as shown in Fig.  6 e.	bind
50389	2	11512	6	10	NULL	0	NULL	statement 1			bind		specifically					putative		AP2/SP1 site	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_10_7661_s_159	11113118	A nuclear protein isolated from rat gastric corpus also specifically bound to the putative AP2/SP1 site, as shown in Fig.  6 e.	bind
51027	1	11513	5	NULL	NULL	NULL	NULL	SRF	GP		is					serum response factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_407_1_7_s_5	9141471	A nuclear protein termed serum response factor (SRF) binds the CArG box motifs, the inner core of SRE, present in the promoter regions of many immediate early genes including  c-fos and several actins [ 1,   3].	bind
51028	2	11513	5	NULL	NULL	NULL	NULL	SRF	GP		is a type of					nuclear protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_407_1_7_s_5	9141471	A nuclear protein termed serum response factor (SRF) binds the CArG box motifs, the inner core of SRE, present in the promoter regions of many immediate early genes including  c-fos and several actins [ 1,   3].	bind
51029	3	11513	5	NULL	NULL	NULL	NULL	SRF	GP		bind									CArG box motifs	NULL		NULL	NULL	NULL	NULL	gw60_febslett_407_1_7_s_5	9141471	A nuclear protein termed serum response factor (SRF) binds the CArG box motifs, the inner core of SRE, present in the promoter regions of many immediate early genes including  c-fos and several actins [ 1,   3].	bind
51030	4	11513	5	NULL	NULL	NULL	NULL	SRF	GP		bind									inner core of SRE	NULL		NULL	NULL	NULL	NULL	gw60_febslett_407_1_7_s_5	9141471	A nuclear protein termed serum response factor (SRF) binds the CArG box motifs, the inner core of SRE, present in the promoter regions of many immediate early genes including  c-fos and several actins [ 1,   3].	bind
51031	5	11513	5	NULL	NULL	NULL	NULL	c-fos	GP		is a type of					immediate early genes	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_407_1_7_s_5	9141471	A nuclear protein termed serum response factor (SRF) binds the CArG box motifs, the inner core of SRE, present in the promoter regions of many immediate early genes including  c-fos and several actins [ 1,   3].	bind
51032	6	11513	5	NULL	NULL	NULL	NULL				is present in				CArG box motifs	c-fos	GP			promoter regions	NULL		NULL	NULL	NULL	NULL	gw60_febslett_407_1_7_s_5	9141471	A nuclear protein termed serum response factor (SRF) binds the CArG box motifs, the inner core of SRE, present in the promoter regions of many immediate early genes including  c-fos and several actins [ 1,   3].	bind
51033	7	11513	5	NULL	NULL	NULL	NULL				is present in				inner core of SRE	c-fos	GP			promoter region	NULL		NULL	NULL	NULL	NULL	gw60_febslett_407_1_7_s_5	9141471	A nuclear protein termed serum response factor (SRF) binds the CArG box motifs, the inner core of SRE, present in the promoter regions of many immediate early genes including  c-fos and several actins [ 1,   3].	bind
58809	8	11513	5	NULL	NULL	NULL	NULL				present in				CArG box motifs	actins	GP			promoter region	NULL		NULL	NULL	NULL	NULL	gw60_febslett_407_1_7_s_5	9141471	A nuclear protein termed serum response factor (SRF) binds the CArG box motifs, the inner core of SRE, present in the promoter regions of many immediate early genes including  c-fos and several actins [ 1,   3].	bind
58810	9	11513	5	NULL	NULL	NULL	NULL				present in				inner core of SRE	actins	GP			promoter region	NULL		NULL	NULL	NULL	NULL	gw60_febslett_407_1_7_s_5	9141471	A nuclear protein termed serum response factor (SRF) binds the CArG box motifs, the inner core of SRE, present in the promoter regions of many immediate early genes including  c-fos and several actins [ 1,   3].	bind
50516	1	11513	6	10	NULL	0	NULL	SRF			bind									CArG box motif 	NULL		NULL	NULL	NULL	NULL	gw60_febslett_407_1_7_s_5	9141471	A nuclear protein termed serum response factor (SRF) binds the CArG box motifs, the inner core of SRE, present in the promoter regions of many immediate early genes including  c-fos and several actins [ 1,   3].	bind
50517	2	11513	6	10	NULL	0	NULL	SRF			bind									inner core of SRE 	NULL		NULL	NULL	NULL	NULL	gw60_febslett_407_1_7_s_5	9141471	A nuclear protein termed serum response factor (SRF) binds the CArG box motifs, the inner core of SRE, present in the promoter regions of many immediate early genes including  c-fos and several actins [ 1,   3].	bind
50518	3	11513	6	NULL	NULL	0	NULL	SRF	NULL		is	NULL				serum response factor	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_407_1_7_s_5	9141471	A nuclear protein termed serum response factor (SRF) binds the CArG box motifs, the inner core of SRE, present in the promoter regions of many immediate early genes including  c-fos and several actins [ 1,   3].	bind
50519	4	11513	6	NULL	NULL	0	NULL	c-fos	NULL		is a type of	NULL				immediate early gene	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_407_1_7_s_5	9141471	A nuclear protein termed serum response factor (SRF) binds the CArG box motifs, the inner core of SRE, present in the promoter regions of many immediate early genes including  c-fos and several actins [ 1,   3].	bind
54158	5	11513	6	10	NULL	0	NULL	SRF			is a type of					nuclear protein					NULL		0	NULL	NULL	NULL	gw60_febslett_407_1_7_s_5	9141471	A nuclear protein termed serum response factor (SRF) binds the CArG box motifs, the inner core of SRE, present in the promoter regions of many immediate early genes including  c-fos and several actins [ 1,   3].	bind
58811	6	11513	6	10	NULL	0	NULL				present in				CArG box motifs	c-fos				promoter region	NULL		NULL	NULL	NULL	NULL	gw60_febslett_407_1_7_s_5	9141471	A nuclear protein termed serum response factor (SRF) binds the CArG box motifs, the inner core of SRE, present in the promoter regions of many immediate early genes including  c-fos and several actins [ 1,   3].	bind
58812	7	11513	6	10	NULL	0	NULL				present in				inner core of SRE	c-fos				promoter region	NULL		NULL	NULL	NULL	NULL	gw60_febslett_407_1_7_s_5	9141471	A nuclear protein termed serum response factor (SRF) binds the CArG box motifs, the inner core of SRE, present in the promoter regions of many immediate early genes including  c-fos and several actins [ 1,   3].	bind
58813	8	11513	6	10	NULL	0	NULL				present in				CArG box motifs	actins				promoter region	NULL		NULL	NULL	NULL	NULL	gw60_febslett_407_1_7_s_5	9141471	A nuclear protein termed serum response factor (SRF) binds the CArG box motifs, the inner core of SRE, present in the promoter regions of many immediate early genes including  c-fos and several actins [ 1,   3].	bind
58814	9	11513	6	10	NULL	0	NULL				present in				inner core of SRE	actins				promoter region	NULL		NULL	NULL	NULL	NULL	gw60_febslett_407_1_7_s_5	9141471	A nuclear protein termed serum response factor (SRF) binds the CArG box motifs, the inner core of SRE, present in the promoter regions of many immediate early genes including  c-fos and several actins [ 1,   3].	bind
51034	1	11514	5	NULL	NULL	NULL	NULL	nuclear protein	GP		bind		specifically			transposons	GP	maize			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_mol-gen-genet_263_3_10821183_s_1	10821183	A nuclear protein that binds specifically to several maize transposons is not essential for Ds1 excision..	bind
51035	2	11514	5	NULL	NULL	NULL	NULL	statement 1	Process		is not essential for					Ds1	GP	excision of			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_mol-gen-genet_263_3_10821183_s_1	10821183	A nuclear protein that binds specifically to several maize transposons is not essential for Ds1 excision..	bind
50390	1	11514	6	NULL	NULL	0	NULL	nuclear protein	NULL		bind	NULL	specifically			transposons	NULL	Maize			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_mol-gen-genet_263_3_10821183_s_1	10821183	A nuclear protein that binds specifically to several maize transposons is not essential for Ds1 excision..	bind
50391	2	11514	6	NULL	NULL	0	NULL	nuclear protein	NULL		is not essential for	NULL				Ds1	NULL	excision of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_mol-gen-genet_263_3_10821183_s_1	10821183	A nuclear protein that binds specifically to several maize transposons is not essential for Ds1 excision..	bind
51036	1	11517	5	NULL	NULL	NULL	NULL	Sos1	GP		is a type of					Ras nucleotide exchange factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20832_s_245	7657668	A number of  SH3-binding proteins have been identified, including the Ras nucleotide  exchange factor Sos1, which binds the SH2- and SH3-containing adaptor  protein Grb-2( 38,  39,  40) ; 3BP1 and 3BP2,  proteins of unknown function that bind the SH3 domain of the c-Abl  tyrosine kinase( 41,  42) ; dynamin, which binds a  variety of SH3 domains ( 43) ; and the GTPase activating protein  CDC42, which binds the SH3 domains of Src and phosphatidylinositol  3-kinase( 44) .	bind
51037	2	11517	5	NULL	NULL	NULL	NULL	Sos1	GP		bind					Grb-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20832_s_245	7657668	A number of  SH3-binding proteins have been identified, including the Ras nucleotide  exchange factor Sos1, which binds the SH2- and SH3-containing adaptor  protein Grb-2( 38,  39,  40) ; 3BP1 and 3BP2,  proteins of unknown function that bind the SH3 domain of the c-Abl  tyrosine kinase( 41,  42) ; dynamin, which binds a  variety of SH3 domains ( 43) ; and the GTPase activating protein  CDC42, which binds the SH3 domains of Src and phosphatidylinositol  3-kinase( 44) .	bind
51038	3	11517	5	NULL	NULL	NULL	NULL	Grb-2	GP		is a type of					adaptor protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20832_s_245	7657668	A number of  SH3-binding proteins have been identified, including the Ras nucleotide  exchange factor Sos1, which binds the SH2- and SH3-containing adaptor  protein Grb-2( 38,  39,  40) ; 3BP1 and 3BP2,  proteins of unknown function that bind the SH3 domain of the c-Abl  tyrosine kinase( 41,  42) ; dynamin, which binds a  variety of SH3 domains ( 43) ; and the GTPase activating protein  CDC42, which binds the SH3 domains of Src and phosphatidylinositol  3-kinase( 44) .	bind
51039	4	11517	5	NULL	NULL	NULL	NULL	3BP1 protein	GP		bind					c-Abl	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20832_s_245	7657668	A number of  SH3-binding proteins have been identified, including the Ras nucleotide  exchange factor Sos1, which binds the SH2- and SH3-containing adaptor  protein Grb-2( 38,  39,  40) ; 3BP1 and 3BP2,  proteins of unknown function that bind the SH3 domain of the c-Abl  tyrosine kinase( 41,  42) ; dynamin, which binds a  variety of SH3 domains ( 43) ; and the GTPase activating protein  CDC42, which binds the SH3 domains of Src and phosphatidylinositol  3-kinase( 44) .	bind
51040	5	11517	5	NULL	NULL	NULL	NULL	c-Abl	GP		is a type of					tyrosine kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20832_s_245	7657668	A number of  SH3-binding proteins have been identified, including the Ras nucleotide  exchange factor Sos1, which binds the SH2- and SH3-containing adaptor  protein Grb-2( 38,  39,  40) ; 3BP1 and 3BP2,  proteins of unknown function that bind the SH3 domain of the c-Abl  tyrosine kinase( 41,  42) ; dynamin, which binds a  variety of SH3 domains ( 43) ; and the GTPase activating protein  CDC42, which binds the SH3 domains of Src and phosphatidylinositol  3-kinase( 44) .	bind
51041	6	11517	5	NULL	NULL	NULL	NULL	3BP2 protein	GP		bind					c-Abl	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20832_s_245	7657668	A number of  SH3-binding proteins have been identified, including the Ras nucleotide  exchange factor Sos1, which binds the SH2- and SH3-containing adaptor  protein Grb-2( 38,  39,  40) ; 3BP1 and 3BP2,  proteins of unknown function that bind the SH3 domain of the c-Abl  tyrosine kinase( 41,  42) ; dynamin, which binds a  variety of SH3 domains ( 43) ; and the GTPase activating protein  CDC42, which binds the SH3 domains of Src and phosphatidylinositol  3-kinase( 44) .	bind
51042	7	11517	5	NULL	NULL	NULL	NULL	dynamin	GP		bind								SH3 domains		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20832_s_245	7657668	A number of  SH3-binding proteins have been identified, including the Ras nucleotide  exchange factor Sos1, which binds the SH2- and SH3-containing adaptor  protein Grb-2( 38,  39,  40) ; 3BP1 and 3BP2,  proteins of unknown function that bind the SH3 domain of the c-Abl  tyrosine kinase( 41,  42) ; dynamin, which binds a  variety of SH3 domains ( 43) ; and the GTPase activating protein  CDC42, which binds the SH3 domains of Src and phosphatidylinositol  3-kinase( 44) .	bind
51043	8	11517	5	NULL	NULL	NULL	NULL	CDC42	GP		is a type of					GTPase activating protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20832_s_245	7657668	A number of  SH3-binding proteins have been identified, including the Ras nucleotide  exchange factor Sos1, which binds the SH2- and SH3-containing adaptor  protein Grb-2( 38,  39,  40) ; 3BP1 and 3BP2,  proteins of unknown function that bind the SH3 domain of the c-Abl  tyrosine kinase( 41,  42) ; dynamin, which binds a  variety of SH3 domains ( 43) ; and the GTPase activating protein  CDC42, which binds the SH3 domains of Src and phosphatidylinositol  3-kinase( 44) .	bind
51044	9	11517	5	NULL	NULL	NULL	NULL	CDC42	GP		bind					Src	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20832_s_245	7657668	A number of  SH3-binding proteins have been identified, including the Ras nucleotide  exchange factor Sos1, which binds the SH2- and SH3-containing adaptor  protein Grb-2( 38,  39,  40) ; 3BP1 and 3BP2,  proteins of unknown function that bind the SH3 domain of the c-Abl  tyrosine kinase( 41,  42) ; dynamin, which binds a  variety of SH3 domains ( 43) ; and the GTPase activating protein  CDC42, which binds the SH3 domains of Src and phosphatidylinositol  3-kinase( 44) .	bind
51045	10	11517	5	NULL	NULL	NULL	NULL	CDC42	GP		bind					phosphatidylinositol 3-kinase	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20832_s_245	7657668	A number of  SH3-binding proteins have been identified, including the Ras nucleotide  exchange factor Sos1, which binds the SH2- and SH3-containing adaptor  protein Grb-2( 38,  39,  40) ; 3BP1 and 3BP2,  proteins of unknown function that bind the SH3 domain of the c-Abl  tyrosine kinase( 41,  42) ; dynamin, which binds a  variety of SH3 domains ( 43) ; and the GTPase activating protein  CDC42, which binds the SH3 domains of Src and phosphatidylinositol  3-kinase( 44) .	bind
54159	11	11517	5	NULL	NULL	NULL	NULL	Grb2	GP		contains only								SH2 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20832_s_245	7657668	A number of  SH3-binding proteins have been identified, including the Ras nucleotide  exchange factor Sos1, which binds the SH2- and SH3-containing adaptor  protein Grb-2( 38,  39,  40) ; 3BP1 and 3BP2,  proteins of unknown function that bind the SH3 domain of the c-Abl  tyrosine kinase( 41,  42) ; dynamin, which binds a  variety of SH3 domains ( 43) ; and the GTPase activating protein  CDC42, which binds the SH3 domains of Src and phosphatidylinositol  3-kinase( 44) .	bind
54160	12	11517	5	NULL	NULL	NULL	NULL	Grb2	GP		contains 								SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20832_s_245	7657668	A number of  SH3-binding proteins have been identified, including the Ras nucleotide  exchange factor Sos1, which binds the SH2- and SH3-containing adaptor  protein Grb-2( 38,  39,  40) ; 3BP1 and 3BP2,  proteins of unknown function that bind the SH3 domain of the c-Abl  tyrosine kinase( 41,  42) ; dynamin, which binds a  variety of SH3 domains ( 43) ; and the GTPase activating protein  CDC42, which binds the SH3 domains of Src and phosphatidylinositol  3-kinase( 44) .	bind
50520	1	11517	6	10	NULL	0	NULL	Sos1			is a type of					Ras nucleotide exchange factor					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20832_s_245	7657668	A number of  SH3-binding proteins have been identified, including the Ras nucleotide  exchange factor Sos1, which binds the SH2- and SH3-containing adaptor  protein Grb-2( 38,  39,  40) ; 3BP1 and 3BP2,  proteins of unknown function that bind the SH3 domain of the c-Abl  tyrosine kinase( 41,  42) ; dynamin, which binds a  variety of SH3 domains ( 43) ; and the GTPase activating protein  CDC42, which binds the SH3 domains of Src and phosphatidylinositol  3-kinase( 44) .	bind
50521	2	11517	6	NULL	NULL	0	NULL	Sos1	NULL		bind	NULL				Grb-2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20832_s_245	7657668	A number of  SH3-binding proteins have been identified, including the Ras nucleotide  exchange factor Sos1, which binds the SH2- and SH3-containing adaptor  protein Grb-2( 38,  39,  40) ; 3BP1 and 3BP2,  proteins of unknown function that bind the SH3 domain of the c-Abl  tyrosine kinase( 41,  42) ; dynamin, which binds a  variety of SH3 domains ( 43) ; and the GTPase activating protein  CDC42, which binds the SH3 domains of Src and phosphatidylinositol  3-kinase( 44) .	bind
50522	3	11517	6	NULL	NULL	0	NULL	Grb-2	NULL		is a type of	NULL				adaptor protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20832_s_245	7657668	A number of  SH3-binding proteins have been identified, including the Ras nucleotide  exchange factor Sos1, which binds the SH2- and SH3-containing adaptor  protein Grb-2( 38,  39,  40) ; 3BP1 and 3BP2,  proteins of unknown function that bind the SH3 domain of the c-Abl  tyrosine kinase( 41,  42) ; dynamin, which binds a  variety of SH3 domains ( 43) ; and the GTPase activating protein  CDC42, which binds the SH3 domains of Src and phosphatidylinositol  3-kinase( 44) .	bind
50523	4	11517	6	NULL	NULL	0	NULL	Grb-2	NULL		contains	NULL					NULL		SH2 domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20832_s_245	7657668	A number of  SH3-binding proteins have been identified, including the Ras nucleotide  exchange factor Sos1, which binds the SH2- and SH3-containing adaptor  protein Grb-2( 38,  39,  40) ; 3BP1 and 3BP2,  proteins of unknown function that bind the SH3 domain of the c-Abl  tyrosine kinase( 41,  42) ; dynamin, which binds a  variety of SH3 domains ( 43) ; and the GTPase activating protein  CDC42, which binds the SH3 domains of Src and phosphatidylinositol  3-kinase( 44) .	bind
50525	5	11517	6	NULL	NULL	0	NULL	Grb-2	NULL		contains	NULL					NULL		SH3 domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20832_s_245	7657668	A number of  SH3-binding proteins have been identified, including the Ras nucleotide  exchange factor Sos1, which binds the SH2- and SH3-containing adaptor  protein Grb-2( 38,  39,  40) ; 3BP1 and 3BP2,  proteins of unknown function that bind the SH3 domain of the c-Abl  tyrosine kinase( 41,  42) ; dynamin, which binds a  variety of SH3 domains ( 43) ; and the GTPase activating protein  CDC42, which binds the SH3 domains of Src and phosphatidylinositol  3-kinase( 44) .	bind
50527	6	11517	6	NULL	NULL	0	NULL	3BP1	NULL		bind	NULL				c-Abl	NULL		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_35_20832_s_245	7657668	A number of  SH3-binding proteins have been identified, including the Ras nucleotide  exchange factor Sos1, which binds the SH2- and SH3-containing adaptor  protein Grb-2( 38,  39,  40) ; 3BP1 and 3BP2,  proteins of unknown function that bind the SH3 domain of the c-Abl  tyrosine kinase( 41,  42) ; dynamin, which binds a  variety of SH3 domains ( 43) ; and the GTPase activating protein  CDC42, which binds the SH3 domains of Src and phosphatidylinositol  3-kinase( 44) .	bind
50528	7	11517	6	NULL	NULL	0	NULL	3BP2	NULL		bind	NULL				c-Abl	NULL		SH3 domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20832_s_245	7657668	A number of  SH3-binding proteins have been identified, including the Ras nucleotide  exchange factor Sos1, which binds the SH2- and SH3-containing adaptor  protein Grb-2( 38,  39,  40) ; 3BP1 and 3BP2,  proteins of unknown function that bind the SH3 domain of the c-Abl  tyrosine kinase( 41,  42) ; dynamin, which binds a  variety of SH3 domains ( 43) ; and the GTPase activating protein  CDC42, which binds the SH3 domains of Src and phosphatidylinositol  3-kinase( 44) .	bind
50529	8	11517	6	NULL	NULL	0	NULL	c-Abl	NULL		is a type of	NULL				tyrosine kinase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20832_s_245	7657668	A number of  SH3-binding proteins have been identified, including the Ras nucleotide  exchange factor Sos1, which binds the SH2- and SH3-containing adaptor  protein Grb-2( 38,  39,  40) ; 3BP1 and 3BP2,  proteins of unknown function that bind the SH3 domain of the c-Abl  tyrosine kinase( 41,  42) ; dynamin, which binds a  variety of SH3 domains ( 43) ; and the GTPase activating protein  CDC42, which binds the SH3 domains of Src and phosphatidylinositol  3-kinase( 44) .	bind
50530	9	11517	6	NULL	NULL	0	NULL	dynamin	NULL		bind	NULL					NULL		SH3 domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20832_s_245	7657668	A number of  SH3-binding proteins have been identified, including the Ras nucleotide  exchange factor Sos1, which binds the SH2- and SH3-containing adaptor  protein Grb-2( 38,  39,  40) ; 3BP1 and 3BP2,  proteins of unknown function that bind the SH3 domain of the c-Abl  tyrosine kinase( 41,  42) ; dynamin, which binds a  variety of SH3 domains ( 43) ; and the GTPase activating protein  CDC42, which binds the SH3 domains of Src and phosphatidylinositol  3-kinase( 44) .	bind
50531	10	11517	6	NULL	NULL	0	NULL	CDC42	NULL		is a type of	NULL				GTPase activating protein	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20832_s_245	7657668	A number of  SH3-binding proteins have been identified, including the Ras nucleotide  exchange factor Sos1, which binds the SH2- and SH3-containing adaptor  protein Grb-2( 38,  39,  40) ; 3BP1 and 3BP2,  proteins of unknown function that bind the SH3 domain of the c-Abl  tyrosine kinase( 41,  42) ; dynamin, which binds a  variety of SH3 domains ( 43) ; and the GTPase activating protein  CDC42, which binds the SH3 domains of Src and phosphatidylinositol  3-kinase( 44) .	bind
50532	11	11517	6	NULL	NULL	0	NULL	CDC42	NULL		bind	NULL				Src	NULL		SH3 domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20832_s_245	7657668	A number of  SH3-binding proteins have been identified, including the Ras nucleotide  exchange factor Sos1, which binds the SH2- and SH3-containing adaptor  protein Grb-2( 38,  39,  40) ; 3BP1 and 3BP2,  proteins of unknown function that bind the SH3 domain of the c-Abl  tyrosine kinase( 41,  42) ; dynamin, which binds a  variety of SH3 domains ( 43) ; and the GTPase activating protein  CDC42, which binds the SH3 domains of Src and phosphatidylinositol  3-kinase( 44) .	bind
50533	12	11517	6	NULL	NULL	0	NULL	CDC42	NULL		bind	NULL				phosphatidylinositol 3-kinase	NULL		SH3 domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_35_20832_s_245	7657668	A number of  SH3-binding proteins have been identified, including the Ras nucleotide  exchange factor Sos1, which binds the SH2- and SH3-containing adaptor  protein Grb-2( 38,  39,  40) ; 3BP1 and 3BP2,  proteins of unknown function that bind the SH3 domain of the c-Abl  tyrosine kinase( 41,  42) ; dynamin, which binds a  variety of SH3 domains ( 43) ; and the GTPase activating protein  CDC42, which binds the SH3 domains of Src and phosphatidylinositol  3-kinase( 44) .	bind
51046	1	11518	5	NULL	NULL	NULL	NULL	Groucho/LEs	GP		bind					HES proteins	GP				NULL	Drosophila	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_42_26604_s_170	9334241	A number of  TLE and  HES family members are co-expressed in a variety of tissues and cell lines ( 18,  34,  42,  43), and Groucho/LEs bind to HES proteins in both  Drosophila and mammals ( 10,  12,  40), suggesting that they may be part of the high  Mr complexes that we have detected.	bind
51047	2	11518	5	NULL	NULL	NULL	NULL	Groucho/LEs	GP		bind					HES proteins	GP				NULL	Mammals	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_42_26604_s_170	9334241	A number of  TLE and  HES family members are co-expressed in a variety of tissues and cell lines ( 18,  34,  42,  43), and Groucho/LEs bind to HES proteins in both  Drosophila and mammals ( 10,  12,  40), suggesting that they may be part of the high  Mr complexes that we have detected.	bind
50392	1	11518	6	10	NULL	0	NULL	Groucho/LEs			bind					HES proteins					NULL	Drosophila	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_42_26604_s_170	9334241	A number of  TLE and  HES family members are co-expressed in a variety of tissues and cell lines ( 18,  34,  42,  43), and Groucho/LEs bind to HES proteins in both  Drosophila and mammals ( 10,  12,  40), suggesting that they may be part of the high  Mr complexes that we have detected.	bind
54162	2	11518	6	10	NULL	0	NULL	Groucho/LEs			bind					HES proteins					NULL	mammals	0	NULL	NULL	NULL	gw60_jbiolchem_272_42_26604_s_170	9334241	A number of  TLE and  HES family members are co-expressed in a variety of tissues and cell lines ( 18,  34,  42,  43), and Groucho/LEs bind to HES proteins in both  Drosophila and mammals ( 10,  12,  40), suggesting that they may be part of the high  Mr complexes that we have detected.	bind
51048	1	11521	5	NULL	NULL	NULL	NULL	(TORC) 1	GP		activates					PGC-1alpha	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_39_14379_s_4	16980408	A number of activators of PGC-1alpha transcription were found; the most potent activator was the transducer of regulated CREB (cAMP response element-binding protein) binding protein (TORC) 1, a coactivator of CREB.	bind
51049	2	11521	5	NULL	NULL	NULL	NULL	(TORC) 1	GP		is					transducer of regulated CREB binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_39_14379_s_4	16980408	A number of activators of PGC-1alpha transcription were found; the most potent activator was the transducer of regulated CREB (cAMP response element-binding protein) binding protein (TORC) 1, a coactivator of CREB.	bind
51050	3	11521	5	NULL	NULL	NULL	NULL	CREB	GP		is					cAMP response element-binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_39_14379_s_4	16980408	A number of activators of PGC-1alpha transcription were found; the most potent activator was the transducer of regulated CREB (cAMP response element-binding protein) binding protein (TORC) 1, a coactivator of CREB.	bind
51051	4	11521	5	NULL	NULL	NULL	NULL	(TORC) 1	GP		is a coactivator of					CREB	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_39_14379_s_4	16980408	A number of activators of PGC-1alpha transcription were found; the most potent activator was the transducer of regulated CREB (cAMP response element-binding protein) binding protein (TORC) 1, a coactivator of CREB.	bind
50534	1	11521	6	10	NULL	0	NULL	(TORC)1			is a coactivator of					CREB					NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_39_14379_s_4	16980408	A number of activators of PGC-1alpha transcription were found; the most potent activator was the transducer of regulated CREB (cAMP response element-binding protein) binding protein (TORC) 1, a coactivator of CREB.	bind
50535	2	11521	6	10	NULL	0	NULL	(TORC)1			activates					PGC-1alpha		transcription of 			NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_39_14379_s_4	16980408	A number of activators of PGC-1alpha transcription were found; the most potent activator was the transducer of regulated CREB (cAMP response element-binding protein) binding protein (TORC) 1, a coactivator of CREB.	bind
50536	3	11521	6	10	NULL	0	NULL	(TORC)1			is					transducer of regulated CREB					NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_39_14379_s_4	16980408	A number of activators of PGC-1alpha transcription were found; the most potent activator was the transducer of regulated CREB (cAMP response element-binding protein) binding protein (TORC) 1, a coactivator of CREB.	bind
50537	4	11521	6	NULL	NULL	0	NULL	CREB	NULL		is	NULL				cAMP response element-binding protein	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_103_39_14379_s_4	16980408	A number of activators of PGC-1alpha transcription were found; the most potent activator was the transducer of regulated CREB (cAMP response element-binding protein) binding protein (TORC) 1, a coactivator of CREB.	bind
51055	1	11522	5	NULL	NULL	NULL	NULL	PCBP2	GP		bind					IRES	GP	polio virus			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_2_639_s_23	12527772	A number of additional viral IRES binding/activating proteins have been identified, including the La autoantigen which is used by polio virus IRES ( 21), and poly r(C) binding protein 2 (PCBP2) which binds to polio virus IRES ( 22) and has been shown to activate entero/rhino virus IRESs  in vitro ( 23).	bind
51056	2	11522	5	NULL	NULL	NULL	NULL	PCBP2	GP		is					poly r(C) binding protein 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_2_639_s_23	12527772	A number of additional viral IRES binding/activating proteins have been identified, including the La autoantigen which is used by polio virus IRES ( 21), and poly r(C) binding protein 2 (PCBP2) which binds to polio virus IRES ( 22) and has been shown to activate entero/rhino virus IRESs  in vitro ( 23).	bind
51057	3	11522	5	NULL	NULL	NULL	NULL	PCBP2	GP		activates					IRES	GP	entero/rhino virus			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_2_639_s_23	12527772	A number of additional viral IRES binding/activating proteins have been identified, including the La autoantigen which is used by polio virus IRES ( 21), and poly r(C) binding protein 2 (PCBP2) which binds to polio virus IRES ( 22) and has been shown to activate entero/rhino virus IRESs  in vitro ( 23).	bind
50393	1	11522	6	NULL	NULL	0	NULL	PCBP2	NULL		bind	NULL				IRES	NULL	polio virus			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_2_639_s_23	12527772	A number of additional viral IRES binding/activating proteins have been identified, including the La autoantigen which is used by polio virus IRES ( 21), and poly r(C) binding protein 2 (PCBP2) which binds to polio virus IRES ( 22) and has been shown to activate entero/rhino virus IRESs  in vitro ( 23).	bind
50394	2	11522	6	NULL	NULL	0	NULL	PCBP2	NULL		is	NULL				poly r(C) binding protein 2	NULL				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_2_639_s_23	12527772	A number of additional viral IRES binding/activating proteins have been identified, including the La autoantigen which is used by polio virus IRES ( 21), and poly r(C) binding protein 2 (PCBP2) which binds to polio virus IRES ( 22) and has been shown to activate entero/rhino virus IRESs  in vitro ( 23).	bind
50395	3	11522	6	NULL	NULL	0	NULL	PCBP2	NULL		activates	NULL				IRES	NULL	entero/rhino virus			NULL	in vitro	0	NULL	NULL	NULL	gw60_nucleicacidsres_31_2_639_s_23	12527772	A number of additional viral IRES binding/activating proteins have been identified, including the La autoantigen which is used by polio virus IRES ( 21), and poly r(C) binding protein 2 (PCBP2) which binds to polio virus IRES ( 22) and has been shown to activate entero/rhino virus IRESs  in vitro ( 23).	bind
51058	1	11526	5	NULL	NULL	NULL	NULL	apoB sequences	AminoAcid		bind		noncovalently			apo(a)	GP				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_45_12_2227_s_26	15375179	A number of apoB sequences that noncovalently bind apo(a) have been reported.	bind
50396	1	11526	6	NULL	NULL	0	NULL	apoB sequences	NULL		bind	NULL	noncovalently			apo(a)	NULL				NULL		0	NULL	NULL	NULL	gw70_jlipidres_45_12_2227_s_26	15375179	A number of apoB sequences that noncovalently bind apo(a) have been reported.	bind
51059	1	11527	5	NULL	NULL	NULL	NULL	HSP47	GP		bind					collagen triple helix	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_38_35007_s_169	12114508	A number of approaches have been used recently to evaluate the binding of HSP47 to the collagen triple helix ( 12,  13).	bind
50397	1	11527	6	NULL	NULL	0	NULL	HSP47	NULL		bind	NULL				collagen triple helix	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_38_35007_s_169	12114508	A number of approaches have been used recently to evaluate the binding of HSP47 to the collagen triple helix ( 12,  13).	bind
51060	1	11528	5	NULL	NULL	NULL	NULL	PDZ45	GP		bind					GluR2 peptide	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_46_43216_s_131	11553623	A number of backbone amide resonances of PDZ45 experienced peptide-induced chemical shift changes in the overlay plot of the 1H-15N HSQC spectra of free PDZ45 ( black) and PDZ45 saturated with the 10-residue GluR2 peptide ( red), indicating that PDZ45 binds to the GluR2 peptide (Fig.  4 B).	bind
50398	1	11528	6	NULL	NULL	0	NULL	PDZ45	NULL		bind	NULL				GluR2 peptide	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_46_43216_s_131	11553623	A number of backbone amide resonances of PDZ45 experienced peptide-induced chemical shift changes in the overlay plot of the 1H-15N HSQC spectra of free PDZ45 ( black) and PDZ45 saturated with the 10-residue GluR2 peptide ( red), indicating that PDZ45 binds to the GluR2 peptide (Fig.  4 B).	bind
51061	1	11529	5	NULL	NULL	NULL	NULL	Bordetella pertussis	Organism		express					outer membrane proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_8_3656_s_22	9673246	A number of bacterial species, including  Bordetella pertussis ( 22),  Helicobacter pylori ( 9),  M. catarrhalis ( 33),  Neisseria gonorrhoeae ( 1),  Neisseria meningitidis ( 29,  33),  Prevotella nigrescens ( 8), and  Treponema spp. ( 34), have been shown to express outer membrane proteins which specifically bind human lactoferrin.	bind
51062	2	11529	5	NULL	NULL	NULL	NULL	statement 1	Process		bind		specifically			lactoferrin	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_8_3656_s_22	9673246	A number of bacterial species, including  Bordetella pertussis ( 22),  Helicobacter pylori ( 9),  M. catarrhalis ( 33),  Neisseria gonorrhoeae ( 1),  Neisseria meningitidis ( 29,  33),  Prevotella nigrescens ( 8), and  Treponema spp. ( 34), have been shown to express outer membrane proteins which specifically bind human lactoferrin.	bind
51063	3	11529	5	NULL	NULL	NULL	NULL	Helicobacter pylori	Organism		express					outer membrane proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_8_3656_s_22	9673246	A number of bacterial species, including  Bordetella pertussis ( 22),  Helicobacter pylori ( 9),  M. catarrhalis ( 33),  Neisseria gonorrhoeae ( 1),  Neisseria meningitidis ( 29,  33),  Prevotella nigrescens ( 8), and  Treponema spp. ( 34), have been shown to express outer membrane proteins which specifically bind human lactoferrin.	bind
51064	4	11529	5	NULL	NULL	NULL	NULL	statement 3	Process		bind		specifically			lactoferrin	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_8_3656_s_22	9673246	A number of bacterial species, including  Bordetella pertussis ( 22),  Helicobacter pylori ( 9),  M. catarrhalis ( 33),  Neisseria gonorrhoeae ( 1),  Neisseria meningitidis ( 29,  33),  Prevotella nigrescens ( 8), and  Treponema spp. ( 34), have been shown to express outer membrane proteins which specifically bind human lactoferrin.	bind
51065	5	11529	5	NULL	NULL	NULL	NULL	M. catarrhalis	Organism		express					outer membrane proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_8_3656_s_22	9673246	A number of bacterial species, including  Bordetella pertussis ( 22),  Helicobacter pylori ( 9),  M. catarrhalis ( 33),  Neisseria gonorrhoeae ( 1),  Neisseria meningitidis ( 29,  33),  Prevotella nigrescens ( 8), and  Treponema spp. ( 34), have been shown to express outer membrane proteins which specifically bind human lactoferrin.	bind
51066	6	11529	5	NULL	NULL	NULL	NULL	statement 5	Process		bind		specifically			lactoferrin	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_8_3656_s_22	9673246	A number of bacterial species, including  Bordetella pertussis ( 22),  Helicobacter pylori ( 9),  M. catarrhalis ( 33),  Neisseria gonorrhoeae ( 1),  Neisseria meningitidis ( 29,  33),  Prevotella nigrescens ( 8), and  Treponema spp. ( 34), have been shown to express outer membrane proteins which specifically bind human lactoferrin.	bind
51067	7	11529	5	NULL	NULL	NULL	NULL	Neisseria gonorrhoeae	Organism		express					outer membrane proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_8_3656_s_22	9673246	A number of bacterial species, including  Bordetella pertussis ( 22),  Helicobacter pylori ( 9),  M. catarrhalis ( 33),  Neisseria gonorrhoeae ( 1),  Neisseria meningitidis ( 29,  33),  Prevotella nigrescens ( 8), and  Treponema spp. ( 34), have been shown to express outer membrane proteins which specifically bind human lactoferrin.	bind
51068	8	11529	5	NULL	NULL	NULL	NULL	statement 7	Process		bind		specifically			lactoferrin	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_8_3656_s_22	9673246	A number of bacterial species, including  Bordetella pertussis ( 22),  Helicobacter pylori ( 9),  M. catarrhalis ( 33),  Neisseria gonorrhoeae ( 1),  Neisseria meningitidis ( 29,  33),  Prevotella nigrescens ( 8), and  Treponema spp. ( 34), have been shown to express outer membrane proteins which specifically bind human lactoferrin.	bind
51069	9	11529	5	NULL	NULL	NULL	NULL	Neisseria meningitidis	Organism		express					outer membrane proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_8_3656_s_22	9673246	A number of bacterial species, including  Bordetella pertussis ( 22),  Helicobacter pylori ( 9),  M. catarrhalis ( 33),  Neisseria gonorrhoeae ( 1),  Neisseria meningitidis ( 29,  33),  Prevotella nigrescens ( 8), and  Treponema spp. ( 34), have been shown to express outer membrane proteins which specifically bind human lactoferrin.	bind
51070	10	11529	5	NULL	NULL	NULL	NULL	statement 9	Process		bind		specifically			lactoferrin	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_8_3656_s_22	9673246	A number of bacterial species, including  Bordetella pertussis ( 22),  Helicobacter pylori ( 9),  M. catarrhalis ( 33),  Neisseria gonorrhoeae ( 1),  Neisseria meningitidis ( 29,  33),  Prevotella nigrescens ( 8), and  Treponema spp. ( 34), have been shown to express outer membrane proteins which specifically bind human lactoferrin.	bind
51071	11	11529	5	NULL	NULL	NULL	NULL	Prevotella nigrescens 	Organism		express					outer membrane proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_8_3656_s_22	9673246	A number of bacterial species, including  Bordetella pertussis ( 22),  Helicobacter pylori ( 9),  M. catarrhalis ( 33),  Neisseria gonorrhoeae ( 1),  Neisseria meningitidis ( 29,  33),  Prevotella nigrescens ( 8), and  Treponema spp. ( 34), have been shown to express outer membrane proteins which specifically bind human lactoferrin.	bind
51072	12	11529	5	NULL	NULL	NULL	NULL	statement 11	Process		bind		specifically			lactoferrin	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_8_3656_s_22	9673246	A number of bacterial species, including  Bordetella pertussis ( 22),  Helicobacter pylori ( 9),  M. catarrhalis ( 33),  Neisseria gonorrhoeae ( 1),  Neisseria meningitidis ( 29,  33),  Prevotella nigrescens ( 8), and  Treponema spp. ( 34), have been shown to express outer membrane proteins which specifically bind human lactoferrin.	bind
51073	13	11529	5	NULL	NULL	NULL	NULL	Treponema spp	Organism		express					outer membrane proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_8_3656_s_22	9673246	A number of bacterial species, including  Bordetella pertussis ( 22),  Helicobacter pylori ( 9),  M. catarrhalis ( 33),  Neisseria gonorrhoeae ( 1),  Neisseria meningitidis ( 29,  33),  Prevotella nigrescens ( 8), and  Treponema spp. ( 34), have been shown to express outer membrane proteins which specifically bind human lactoferrin.	bind
51074	14	11529	5	NULL	NULL	NULL	NULL	statement 13	Process		bind		specifically			lactoferrin	GP	human			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_8_3656_s_22	9673246	A number of bacterial species, including  Bordetella pertussis ( 22),  Helicobacter pylori ( 9),  M. catarrhalis ( 33),  Neisseria gonorrhoeae ( 1),  Neisseria meningitidis ( 29,  33),  Prevotella nigrescens ( 8), and  Treponema spp. ( 34), have been shown to express outer membrane proteins which specifically bind human lactoferrin.	bind
50399	1	11529	6	NULL	NULL	0	NULL	Bordetella pertussis	NULL		express	NULL				outer membrane proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_8_3656_s_22	9673246	A number of bacterial species, including  Bordetella pertussis ( 22),  Helicobacter pylori ( 9),  M. catarrhalis ( 33),  Neisseria gonorrhoeae ( 1),  Neisseria meningitidis ( 29,  33),  Prevotella nigrescens ( 8), and  Treponema spp. ( 34), have been shown to express outer membrane proteins which specifically bind human lactoferrin.	bind
50400	2	11529	6	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL	specifically			lactoferrin	NULL	human			NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_8_3656_s_22	9673246	A number of bacterial species, including  Bordetella pertussis ( 22),  Helicobacter pylori ( 9),  M. catarrhalis ( 33),  Neisseria gonorrhoeae ( 1),  Neisseria meningitidis ( 29,  33),  Prevotella nigrescens ( 8), and  Treponema spp. ( 34), have been shown to express outer membrane proteins which specifically bind human lactoferrin.	bind
50401	3	11529	6	NULL	NULL	0	NULL	Helicobacter pylori 	NULL		express	NULL				outer membrane proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_8_3656_s_22	9673246	A number of bacterial species, including  Bordetella pertussis ( 22),  Helicobacter pylori ( 9),  M. catarrhalis ( 33),  Neisseria gonorrhoeae ( 1),  Neisseria meningitidis ( 29,  33),  Prevotella nigrescens ( 8), and  Treponema spp. ( 34), have been shown to express outer membrane proteins which specifically bind human lactoferrin.	bind
50402	4	11529	6	10	NULL	0	NULL	statement 3			bind		specifically			lactoferrin		human			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_66_8_3656_s_22	9673246	A number of bacterial species, including  Bordetella pertussis ( 22),  Helicobacter pylori ( 9),  M. catarrhalis ( 33),  Neisseria gonorrhoeae ( 1),  Neisseria meningitidis ( 29,  33),  Prevotella nigrescens ( 8), and  Treponema spp. ( 34), have been shown to express outer membrane proteins which specifically bind human lactoferrin.	bind
50403	5	11529	6	NULL	NULL	0	NULL	M. catarrhalis	NULL		express	NULL				outer membrane proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_8_3656_s_22	9673246	A number of bacterial species, including  Bordetella pertussis ( 22),  Helicobacter pylori ( 9),  M. catarrhalis ( 33),  Neisseria gonorrhoeae ( 1),  Neisseria meningitidis ( 29,  33),  Prevotella nigrescens ( 8), and  Treponema spp. ( 34), have been shown to express outer membrane proteins which specifically bind human lactoferrin.	bind
50404	6	11529	6	NULL	NULL	0	NULL	statement 5	NULL		bind	NULL	specifically			lactoferrin	NULL	human			NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_8_3656_s_22	9673246	A number of bacterial species, including  Bordetella pertussis ( 22),  Helicobacter pylori ( 9),  M. catarrhalis ( 33),  Neisseria gonorrhoeae ( 1),  Neisseria meningitidis ( 29,  33),  Prevotella nigrescens ( 8), and  Treponema spp. ( 34), have been shown to express outer membrane proteins which specifically bind human lactoferrin.	bind
50405	7	11529	6	NULL	NULL	0	NULL	Neisseria gonorrhoeae	NULL		express	NULL				outer membrane proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_8_3656_s_22	9673246	A number of bacterial species, including  Bordetella pertussis ( 22),  Helicobacter pylori ( 9),  M. catarrhalis ( 33),  Neisseria gonorrhoeae ( 1),  Neisseria meningitidis ( 29,  33),  Prevotella nigrescens ( 8), and  Treponema spp. ( 34), have been shown to express outer membrane proteins which specifically bind human lactoferrin.	bind
50406	8	11529	6	NULL	NULL	0	NULL	statement 7	NULL		bind	NULL	specifically			lactoferrin	NULL	human			NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_8_3656_s_22	9673246	A number of bacterial species, including  Bordetella pertussis ( 22),  Helicobacter pylori ( 9),  M. catarrhalis ( 33),  Neisseria gonorrhoeae ( 1),  Neisseria meningitidis ( 29,  33),  Prevotella nigrescens ( 8), and  Treponema spp. ( 34), have been shown to express outer membrane proteins which specifically bind human lactoferrin.	bind
50407	9	11529	6	NULL	NULL	0	NULL	Neisseria meningitidis	NULL		express	NULL				outer membrane proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_8_3656_s_22	9673246	A number of bacterial species, including  Bordetella pertussis ( 22),  Helicobacter pylori ( 9),  M. catarrhalis ( 33),  Neisseria gonorrhoeae ( 1),  Neisseria meningitidis ( 29,  33),  Prevotella nigrescens ( 8), and  Treponema spp. ( 34), have been shown to express outer membrane proteins which specifically bind human lactoferrin.	bind
50408	10	11529	6	NULL	NULL	0	NULL	statement 9	NULL		express	NULL	specifically			lactoferrin	NULL	human			NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_8_3656_s_22	9673246	A number of bacterial species, including  Bordetella pertussis ( 22),  Helicobacter pylori ( 9),  M. catarrhalis ( 33),  Neisseria gonorrhoeae ( 1),  Neisseria meningitidis ( 29,  33),  Prevotella nigrescens ( 8), and  Treponema spp. ( 34), have been shown to express outer membrane proteins which specifically bind human lactoferrin.	bind
50409	11	11529	6	NULL	NULL	0	NULL	Prevotella nigrescens	NULL		express	NULL				outer membrane proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_8_3656_s_22	9673246	A number of bacterial species, including  Bordetella pertussis ( 22),  Helicobacter pylori ( 9),  M. catarrhalis ( 33),  Neisseria gonorrhoeae ( 1),  Neisseria meningitidis ( 29,  33),  Prevotella nigrescens ( 8), and  Treponema spp. ( 34), have been shown to express outer membrane proteins which specifically bind human lactoferrin.	bind
50410	12	11529	6	NULL	NULL	0	NULL	statement 11	NULL		bind	NULL	specifically			lactoferrin	NULL	human			NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_8_3656_s_22	9673246	A number of bacterial species, including  Bordetella pertussis ( 22),  Helicobacter pylori ( 9),  M. catarrhalis ( 33),  Neisseria gonorrhoeae ( 1),  Neisseria meningitidis ( 29,  33),  Prevotella nigrescens ( 8), and  Treponema spp. ( 34), have been shown to express outer membrane proteins which specifically bind human lactoferrin.	bind
50411	13	11529	6	NULL	NULL	0	NULL	Treponema spp.	NULL		express	NULL				outer membrane proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_8_3656_s_22	9673246	A number of bacterial species, including  Bordetella pertussis ( 22),  Helicobacter pylori ( 9),  M. catarrhalis ( 33),  Neisseria gonorrhoeae ( 1),  Neisseria meningitidis ( 29,  33),  Prevotella nigrescens ( 8), and  Treponema spp. ( 34), have been shown to express outer membrane proteins which specifically bind human lactoferrin.	bind
50412	14	11529	6	NULL	NULL	0	NULL	statement 13	NULL		bind	NULL	specifically			lactoferrin	NULL	human			NULL		0	NULL	NULL	NULL	gw60_infectimmun_66_8_3656_s_22	9673246	A number of bacterial species, including  Bordetella pertussis ( 22),  Helicobacter pylori ( 9),  M. catarrhalis ( 33),  Neisseria gonorrhoeae ( 1),  Neisseria meningitidis ( 29,  33),  Prevotella nigrescens ( 8), and  Treponema spp. ( 34), have been shown to express outer membrane proteins which specifically bind human lactoferrin.	bind
51075	1	11530	5	NULL	NULL	NULL	NULL	GTP-binding proteins	GP	small	bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_3_904_s_138	12538863	A number of bacterial toxins specifically target the GTP-bound form of small GTP-binding proteins ( ,  ).	bind
51076	2	11530	5	NULL	NULL	NULL	NULL	bacterial toxins	GP		targets		specifically			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_3_904_s_138	12538863	A number of bacterial toxins specifically target the GTP-bound form of small GTP-binding proteins ( ,  ).	bind
50413	1	11530	6	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				GTP-binding proteins	NULL	small			NULL		0	NULL	NULL	NULL	gw70_pnas_100_3_904_s_138	12538863	A number of bacterial toxins specifically target the GTP-bound form of small GTP-binding proteins ( ,  ).	bind
50414	2	11530	6	NULL	NULL	0	NULL	bacterial toxins	NULL		target	NULL	specifically			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_100_3_904_s_138	12538863	A number of bacterial toxins specifically target the GTP-bound form of small GTP-binding proteins ( ,  ).	bind
51077	1	11533	5	NULL	NULL	NULL	NULL	catenins	GP		bind		directly			cadherin	GP		cytoplasmic tails		NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_275_39_10899158_s_3	10899158	A number of catenins directly bind cadherin cytoplasmic tails, contributing  to the modulation of cell-cell adhesion and motility processes.	bind
51078	2	11533	5	NULL	NULL	NULL	NULL	statement 1	Process		contribute to					cell-cell adhesion	Process	modulation of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_275_39_10899158_s_3	10899158	A number of catenins directly bind cadherin cytoplasmic tails, contributing  to the modulation of cell-cell adhesion and motility processes.	bind
51079	3	11533	5	NULL	NULL	NULL	NULL	statement 1	Process		contribute to					cell motility 	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_275_39_10899158_s_3	10899158	A number of catenins directly bind cadherin cytoplasmic tails, contributing  to the modulation of cell-cell adhesion and motility processes.	bind
50415	1	11533	6	NULL	NULL	0	NULL	catenins	NULL		bind	NULL	directly			cadherin	NULL		cytoplasmic tails		NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_275_39_10899158_s_3	10899158	A number of catenins directly bind cadherin cytoplasmic tails, contributing  to the modulation of cell-cell adhesion and motility processes.	bind
50416	2	11533	6	10	NULL	0	NULL	statement 1			contributes to					cell-cell adhesion		modulation of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_275_39_10899158_s_3	10899158	A number of catenins directly bind cadherin cytoplasmic tails, contributing  to the modulation of cell-cell adhesion and motility processes.	bind
50417	3	11533	6	NULL	NULL	0	NULL	statement 1	NULL		contributes to	NULL				cell motility	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_275_39_10899158_s_3	10899158	A number of catenins directly bind cadherin cytoplasmic tails, contributing  to the modulation of cell-cell adhesion and motility processes.	bind
51080	1	11535	5	NULL	NULL	NULL	NULL	LPL	GP		bind					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_41_24525_s_21	7592670	A number of conflicting reports show that binding  of LPL to heparin, a proteoglycan very similar to heparan sulfate, can  stabilize, stimulate, or inhibit catalytic efficiency of the lipase  depending on experimental conditions ( 13,  14,  15,  16) .	bind
51081	2	11535	5	NULL	NULL	NULL	NULL	heparin	Chemical		is a type of					proteoglycan	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_41_24525_s_21	7592670	A number of conflicting reports show that binding  of LPL to heparin, a proteoglycan very similar to heparan sulfate, can  stabilize, stimulate, or inhibit catalytic efficiency of the lipase  depending on experimental conditions ( 13,  14,  15,  16) .	bind
51082	3	11535	5	NULL	NULL	NULL	NULL	heparin	Chemical		is similar to					heparan sulfate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_41_24525_s_21	7592670	A number of conflicting reports show that binding  of LPL to heparin, a proteoglycan very similar to heparan sulfate, can  stabilize, stimulate, or inhibit catalytic efficiency of the lipase  depending on experimental conditions ( 13,  14,  15,  16) .	bind
50418	1	11535	6	NULL	NULL	0	NULL	LPL	NULL		bind	NULL				heparin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_41_24525_s_21	7592670	A number of conflicting reports show that binding  of LPL to heparin, a proteoglycan very similar to heparan sulfate, can  stabilize, stimulate, or inhibit catalytic efficiency of the lipase  depending on experimental conditions ( 13,  14,  15,  16) .	bind
50419	2	11535	6	NULL	NULL	0	NULL	heparin	NULL		is a type of	NULL				proteoglycan	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_41_24525_s_21	7592670	A number of conflicting reports show that binding  of LPL to heparin, a proteoglycan very similar to heparan sulfate, can  stabilize, stimulate, or inhibit catalytic efficiency of the lipase  depending on experimental conditions ( 13,  14,  15,  16) .	bind
50420	3	11535	6	NULL	NULL	0	NULL	heparin	NULL		is similar to	NULL				heparan sulfate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_41_24525_s_21	7592670	A number of conflicting reports show that binding  of LPL to heparin, a proteoglycan very similar to heparan sulfate, can  stabilize, stimulate, or inhibit catalytic efficiency of the lipase  depending on experimental conditions ( 13,  14,  15,  16) .	bind
51083	1	11536	5	NULL	NULL	NULL	NULL	detoxification proteins	GP		bind					thioredoxin	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_11_3759_s_151	15004283	A number of detoxification proteins were found to bind thioredoxin.	bind
50421	1	11536	6	NULL	NULL	0	NULL	detoxification proteins	NULL		bind	NULL				thioredoxin	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_101_11_3759_s_151	15004283	A number of detoxification proteins were found to bind thioredoxin.	bind
51084	1	11537	5	NULL	NULL	NULL	NULL	PAKs	GP		bind		directly			Nck	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_8_6037_s_8	11096073	A number of different functions have been ascribed to PAKs; and PAKs can bind directly to growth factor signaling-adaptor molecule, Nck, and a guanine nucleotide exchanger, betaPIX.	bind
51085	2	11537	5	NULL	NULL	NULL	NULL	PAKs	GP		bind		directly			betaPIX	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_8_6037_s_8	11096073	A number of different functions have been ascribed to PAKs; and PAKs can bind directly to growth factor signaling-adaptor molecule, Nck, and a guanine nucleotide exchanger, betaPIX.	bind
51086	3	11537	5	NULL	NULL	NULL	NULL	Nck	GP		is a type of					growth factor signaling-adaptor molecule	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_8_6037_s_8	11096073	A number of different functions have been ascribed to PAKs; and PAKs can bind directly to growth factor signaling-adaptor molecule, Nck, and a guanine nucleotide exchanger, betaPIX.	bind
51087	4	11537	5	NULL	NULL	NULL	NULL	betaPIX	GP		is a type of					guanine nucleotide exchanger	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_8_6037_s_8	11096073	A number of different functions have been ascribed to PAKs; and PAKs can bind directly to growth factor signaling-adaptor molecule, Nck, and a guanine nucleotide exchanger, betaPIX.	bind
50422	1	11537	6	NULL	NULL	0	NULL	PAK	NULL		bind	NULL	directly			Nck	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_8_6037_s_8	11096073	A number of different functions have been ascribed to PAKs; and PAKs can bind directly to growth factor signaling-adaptor molecule, Nck, and a guanine nucleotide exchanger, betaPIX.	bind
50423	2	11537	6	NULL	NULL	0	NULL	Nck	NULL		is a type of	NULL				growth factor signaling-adaptor molecule	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_8_6037_s_8	11096073	A number of different functions have been ascribed to PAKs; and PAKs can bind directly to growth factor signaling-adaptor molecule, Nck, and a guanine nucleotide exchanger, betaPIX.	bind
50424	3	11537	6	NULL	NULL	0	NULL	PAK	NULL		bind	NULL	directly			betaPIX	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_8_6037_s_8	11096073	A number of different functions have been ascribed to PAKs; and PAKs can bind directly to growth factor signaling-adaptor molecule, Nck, and a guanine nucleotide exchanger, betaPIX.	bind
50425	4	11537	6	NULL	NULL	0	NULL	betaPIX	NULL		is a type of	NULL				guanine nucleotide exchanger	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_8_6037_s_8	11096073	A number of different functions have been ascribed to PAKs; and PAKs can bind directly to growth factor signaling-adaptor molecule, Nck, and a guanine nucleotide exchanger, betaPIX.	bind
51088	1	11539	5	NULL	NULL	NULL	NULL	PI lipids	Chemical		bind					AP-2	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_21_1383_s_85	11084340	A number of different PI lipids bind the adaptor protein complex AP-2, facilitating its self-assembly, and its interaction with clathrin and peptides that contain endocytic motifs  [8  .	bind
51089	2	11539	5	NULL	NULL	NULL	NULL	AP-2	GP		is a type of					adaptor protein complex	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_21_1383_s_85	11084340	A number of different PI lipids bind the adaptor protein complex AP-2, facilitating its self-assembly, and its interaction with clathrin and peptides that contain endocytic motifs  [8  .	bind
51090	3	11539	5	NULL	NULL	NULL	NULL	statement 1	Process		facilitates					AP-2	GP	self-assembly of			NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_21_1383_s_85	11084340	A number of different PI lipids bind the adaptor protein complex AP-2, facilitating its self-assembly, and its interaction with clathrin and peptides that contain endocytic motifs  [8  .	bind
51091	4	11539	5	NULL	NULL	NULL	NULL	AP-2	GP		interacts with					clathrin	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_21_1383_s_85	11084340	A number of different PI lipids bind the adaptor protein complex AP-2, facilitating its self-assembly, and its interaction with clathrin and peptides that contain endocytic motifs  [8  .	bind
51092	5	11539	5	NULL	NULL	NULL	NULL	peptides	AminoAcid		contains								endocytic motifs		NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_21_1383_s_85	11084340	A number of different PI lipids bind the adaptor protein complex AP-2, facilitating its self-assembly, and its interaction with clathrin and peptides that contain endocytic motifs  [8  .	bind
51093	6	11539	5	NULL	NULL	NULL	NULL	AP-2	GP		interacts with					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_21_1383_s_85	11084340	A number of different PI lipids bind the adaptor protein complex AP-2, facilitating its self-assembly, and its interaction with clathrin and peptides that contain endocytic motifs  [8  .	bind
51094	7	11539	5	NULL	NULL	NULL	NULL	statement 1	Process		facilitates					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_21_1383_s_85	11084340	A number of different PI lipids bind the adaptor protein complex AP-2, facilitating its self-assembly, and its interaction with clathrin and peptides that contain endocytic motifs  [8  .	bind
51095	8	11539	5	NULL	NULL	NULL	NULL	statement 1	Process		facilitates					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_21_1383_s_85	11084340	A number of different PI lipids bind the adaptor protein complex AP-2, facilitating its self-assembly, and its interaction with clathrin and peptides that contain endocytic motifs  [8  .	bind
50426	1	11539	6	NULL	NULL	0	NULL	PI lipids	NULL		bind	NULL				AP-2	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_21_1383_s_85	11084340	A number of different PI lipids bind the adaptor protein complex AP-2, facilitating its self-assembly, and its interaction with clathrin and peptides that contain endocytic motifs  [8  .	bind
50427	2	11539	6	NULL	NULL	0	NULL	AP-2	NULL		is a type of	NULL				adaptor protein complex	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_21_1383_s_85	11084340	A number of different PI lipids bind the adaptor protein complex AP-2, facilitating its self-assembly, and its interaction with clathrin and peptides that contain endocytic motifs  [8  .	bind
50428	3	11539	6	NULL	NULL	0	NULL	statement 1	NULL		facilitates	NULL				AP-2	NULL	self assembly of 			NULL		0	NULL	NULL	NULL	gw60_currbiol_10_21_1383_s_85	11084340	A number of different PI lipids bind the adaptor protein complex AP-2, facilitating its self-assembly, and its interaction with clathrin and peptides that contain endocytic motifs  [8  .	bind
50429	4	11539	6	NULL	NULL	0	NULL	AP-2	NULL		interacts with	NULL				clathrin	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_21_1383_s_85	11084340	A number of different PI lipids bind the adaptor protein complex AP-2, facilitating its self-assembly, and its interaction with clathrin and peptides that contain endocytic motifs  [8  .	bind
50430	5	11539	6	NULL	NULL	0	NULL	peptides	NULL		contain	NULL					NULL		endocytic motifs		NULL		0	NULL	NULL	NULL	gw60_currbiol_10_21_1383_s_85	11084340	A number of different PI lipids bind the adaptor protein complex AP-2, facilitating its self-assembly, and its interaction with clathrin and peptides that contain endocytic motifs  [8  .	bind
50431	6	11539	6	NULL	NULL	0	NULL	AP-2	NULL		interacts with	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_21_1383_s_85	11084340	A number of different PI lipids bind the adaptor protein complex AP-2, facilitating its self-assembly, and its interaction with clathrin and peptides that contain endocytic motifs  [8  .	bind
54163	7	11539	6	10	NULL	0	NULL	statement 1			facilitate					statement 4					NULL		0	NULL	NULL	NULL	gw60_currbiol_10_21_1383_s_85	11084340	A number of different PI lipids bind the adaptor protein complex AP-2, facilitating its self-assembly, and its interaction with clathrin and peptides that contain endocytic motifs  [8  .	bind
54164	8	11539	6	10	NULL	0	NULL	statement 1			facilitate					statement 6					NULL		0	NULL	NULL	NULL	gw60_currbiol_10_21_1383_s_85	11084340	A number of different PI lipids bind the adaptor protein complex AP-2, facilitating its self-assembly, and its interaction with clathrin and peptides that contain endocytic motifs  [8  .	bind
51096	1	11540	5	NULL	NULL	NULL	NULL	AP-1	GP		bind					 GADD45 gene	GP			binding site on promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_26_20061_s_248	10751396	A number of DNA-protein interactions, including binding of AP-1 and p53 on their respective binding sites, were required to maintain the poised chromatin structure of the  GADD45 gene promoter ( 47).	bind
51097	2	11540	5	NULL	NULL	NULL	NULL	p53	GP		bind					GADD45 gene 	GP			binding site on promoter	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_26_20061_s_248	10751396	A number of DNA-protein interactions, including binding of AP-1 and p53 on their respective binding sites, were required to maintain the poised chromatin structure of the  GADD45 gene promoter ( 47).	bind
56601	3	11540	5	NULL	NULL	NULL	NULL	statement 1	Process		required for					GADD45 gene 	GP	 poised chromatin structure of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_26_20061_s_248	10751396	A number of DNA-protein interactions, including binding of AP-1 and p53 on their respective binding sites, were required to maintain the poised chromatin structure of the  GADD45 gene promoter ( 47).	bind
56602	4	11540	5	NULL	NULL	NULL	NULL	statement 2	Process		required for					GADD45 gene 	GP	poised chromatin structure of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_26_20061_s_248	10751396	A number of DNA-protein interactions, including binding of AP-1 and p53 on their respective binding sites, were required to maintain the poised chromatin structure of the  GADD45 gene promoter ( 47).	bind
50432	1	11540	6	NULL	NULL	0	NULL	AP-1	NULL		bind	NULL				GADD45 gene	NULL			site on promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_26_20061_s_248	10751396	A number of DNA-protein interactions, including binding of AP-1 and p53 on their respective binding sites, were required to maintain the poised chromatin structure of the  GADD45 gene promoter ( 47).	bind
50433	2	11540	6	NULL	NULL	0	NULL	p53	NULL		bind	NULL				GADD45 gene	NULL			site on promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_26_20061_s_248	10751396	A number of DNA-protein interactions, including binding of AP-1 and p53 on their respective binding sites, were required to maintain the poised chromatin structure of the  GADD45 gene promoter ( 47).	bind
50434	3	11540	6	10	NULL	0	NULL	statement 1			is required for					GADD45 gene 		poised chromatin structure of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_26_20061_s_248	10751396	A number of DNA-protein interactions, including binding of AP-1 and p53 on their respective binding sites, were required to maintain the poised chromatin structure of the  GADD45 gene promoter ( 47).	bind
50435	4	11540	6	10	NULL	0	NULL	statement 2			is required for					GADD45 gene 		poised chromatin structure of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_26_20061_s_248	10751396	A number of DNA-protein interactions, including binding of AP-1 and p53 on their respective binding sites, were required to maintain the poised chromatin structure of the  GADD45 gene promoter ( 47).	bind
51098	1	11541	5	NULL	NULL	NULL	NULL	GTP	Chemical		bind					ARF proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_18_13465_s_275	10788460	A number of effector proteins were found to have the ability to increase the equilibrium level of GTP binding to ARF proteins.	bind
51099	2	11541	5	NULL	NULL	NULL	NULL	effector proteins	GP		increases					statement 1	Process	equilibrium level of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_18_13465_s_275	10788460	A number of effector proteins were found to have the ability to increase the equilibrium level of GTP binding to ARF proteins.	bind
50436	1	11541	6	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				ARF proteins	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13465_s_275	10788460	A number of effector proteins were found to have the ability to increase the equilibrium level of GTP binding to ARF proteins.	bind
54190	2	11541	6	10	NULL	0	NULL	effector proteins			increase					statement 1		equilibrium level of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13465_s_275	10788460	A number of effector proteins were found to have the ability to increase the equilibrium level of GTP binding to ARF proteins.	bind
51100	1	11542	5	NULL	NULL	NULL	NULL	Pumilio	GP		bind									NREs	NULL	embryo	NULL	NULL	NULL	NULL	gw60_genetics_153_4_1825_s_29	10581288	A number of experiments suggest that Pumilio is bound to the NREs throughout the embryo ( M URATA and WHARTON 1995   ;	bind
50437	1	11542	6	10	NULL	0	NULL	Pumilio			bind									NRE	NULL	 embryo	NULL	NULL	NULL	NULL	gw60_genetics_153_4_1825_s_29	10581288	A number of experiments suggest that Pumilio is bound to the NREs throughout the embryo ( M URATA and WHARTON 1995   ;	bind
51101	1	11543	5	NULL	NULL	NULL	NULL	TMR	GP		bind								Cys-374		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_36_34172_s_169	12813032	A number of factors  could help explain this small difference, including the use of AMPPNP in place  of ATP, the binding of TMR to Cys-374, or the fact that this is the first  ATP-actin structure to have been determined without any other protein bound to  it.	bind
50438	1	11543	6	NULL	NULL	0	NULL	TMR	NULL		bind	NULL					NULL		Cys-374		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_36_34172_s_169	12813032	A number of factors  could help explain this small difference, including the use of AMPPNP in place  of ATP, the binding of TMR to Cys-374, or the fact that this is the first  ATP-actin structure to have been determined without any other protein bound to  it.	bind
51102	1	11544	5	NULL	NULL	NULL	NULL	HNF-3	GP		is					hepatic nuclear factor 3	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3446_s_44	10652338	A number of factors bind to gAF2, although only binding of hepatic nuclear factor 3 (HNF-3) specifically correlates with the ability of the gAF2 element to induce the glucocorticoid response ( 28).	bind
51103	2	11544	5	NULL	NULL	NULL	NULL	HNF-3	GP		bind					gAF2	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3446_s_44	10652338	A number of factors bind to gAF2, although only binding of hepatic nuclear factor 3 (HNF-3) specifically correlates with the ability of the gAF2 element to induce the glucocorticoid response ( 28).	bind
51104	3	11544	5	NULL	NULL	NULL	NULL				induce				gAF2 element	glucocorticoid response	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3446_s_44	10652338	A number of factors bind to gAF2, although only binding of hepatic nuclear factor 3 (HNF-3) specifically correlates with the ability of the gAF2 element to induce the glucocorticoid response ( 28).	bind
51105	4	11544	5	NULL	NULL	NULL	NULL	statement 2	Process		corelates with		specifically			statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3446_s_44	10652338	A number of factors bind to gAF2, although only binding of hepatic nuclear factor 3 (HNF-3) specifically correlates with the ability of the gAF2 element to induce the glucocorticoid response ( 28).	bind
50439	1	11544	6	NULL	NULL	0	NULL		NULL		induce	NULL			gAF2 element	glucocorticoid response	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_5_3446_s_44	10652338	A number of factors bind to gAF2, although only binding of hepatic nuclear factor 3 (HNF-3) specifically correlates with the ability of the gAF2 element to induce the glucocorticoid response ( 28).	bind
50440	2	11544	6	10	NULL	0	NULL	HNF-3			bind					gAF2					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3446_s_44	10652338	A number of factors bind to gAF2, although only binding of hepatic nuclear factor 3 (HNF-3) specifically correlates with the ability of the gAF2 element to induce the glucocorticoid response ( 28).	bind
50441	3	11544	6	10	NULL	0	NULL	statement 2			correlates with		specifically			statement 1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3446_s_44	10652338	A number of factors bind to gAF2, although only binding of hepatic nuclear factor 3 (HNF-3) specifically correlates with the ability of the gAF2 element to induce the glucocorticoid response ( 28).	bind
54191	4	11544	6	10	NULL	0	NULL	HNF-3			is					hepatic nuclear factor 3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_5_3446_s_44	10652338	A number of factors bind to gAF2, although only binding of hepatic nuclear factor 3 (HNF-3) specifically correlates with the ability of the gAF2 element to induce the glucocorticoid response ( 28).	bind
51106	1	11545	5	NULL	NULL	NULL	NULL	fibroblast growth factors	GP		bind					tyrosine kinase receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_22_11722_s_31	11050201	A number of fibroblast growth factors that bind and activate tyrosine kinase receptors are known to be present in inner ear organs ( 54,  55).	bind
51107	2	11545	5	NULL	NULL	NULL	NULL	statement 1	Process		activates					tyrosine kinase receptors	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_22_11722_s_31	11050201	A number of fibroblast growth factors that bind and activate tyrosine kinase receptors are known to be present in inner ear organs ( 54,  55).	bind
51108	3	11545	5	NULL	NULL	NULL	NULL	fibroblast growth factors	GP		is present in					inner ear organs	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_22_11722_s_31	11050201	A number of fibroblast growth factors that bind and activate tyrosine kinase receptors are known to be present in inner ear organs ( 54,  55).	bind
50442	1	11545	6	NULL	NULL	0	NULL	fibroblast growth factor	NULL		bind	NULL				tyrosine kinase receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_22_11722_s_31	11050201	A number of fibroblast growth factors that bind and activate tyrosine kinase receptors are known to be present in inner ear organs ( 54,  55).	bind
50443	2	11545	6	NULL	NULL	0	NULL	fibroblast growth factor	NULL		activates	NULL				tyrosine kinase receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_22_11722_s_31	11050201	A number of fibroblast growth factors that bind and activate tyrosine kinase receptors are known to be present in inner ear organs ( 54,  55).	bind
50444	3	11545	6	NULL	NULL	0	NULL	fibroblast growth factor	NULL		are present in	NULL				inner ear organs	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_22_11722_s_31	11050201	A number of fibroblast growth factors that bind and activate tyrosine kinase receptors are known to be present in inner ear organs ( 54,  55).	bind
51109	1	11546	5	NULL	NULL	NULL	NULL	GTP	Chemical		bind					ARF	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_11_3133_s_37	9802902	A number of GEFs, which promote binding of GTP to ARF by facilitating the release of GDP, have been identified (Chardin  et al., 1996  ; Peyroche  et al., 1996  ; Klarlund  et al., 1997  ; Meacci  et al., 1997  ; Morinaga  et al., 1997  ; Sata  et al., 1998  ).	bind
51110	2	11546	5	NULL	NULL	NULL	NULL	GEFs	GP		promotes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_11_3133_s_37	9802902	A number of GEFs, which promote binding of GTP to ARF by facilitating the release of GDP, have been identified (Chardin  et al., 1996  ; Peyroche  et al., 1996  ; Klarlund  et al., 1997  ; Meacci  et al., 1997  ; Morinaga  et al., 1997  ; Sata  et al., 1998  ).	bind
51111	3	11546	5	NULL	NULL	NULL	NULL	GEFs	GP		facilitates					GDP	Chemical	release of			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_11_3133_s_37	9802902	A number of GEFs, which promote binding of GTP to ARF by facilitating the release of GDP, have been identified (Chardin  et al., 1996  ; Peyroche  et al., 1996  ; Klarlund  et al., 1997  ; Meacci  et al., 1997  ; Morinaga  et al., 1997  ; Sata  et al., 1998  ).	bind
51112	4	11546	5	NULL	NULL	NULL	NULL	statement 3	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_9_11_3133_s_37	9802902	A number of GEFs, which promote binding of GTP to ARF by facilitating the release of GDP, have been identified (Chardin  et al., 1996  ; Peyroche  et al., 1996  ; Klarlund  et al., 1997  ; Meacci  et al., 1997  ; Morinaga  et al., 1997  ; Sata  et al., 1998  ).	bind
50445	1	11546	6	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				ARF	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_9_11_3133_s_37	9802902	A number of GEFs, which promote binding of GTP to ARF by facilitating the release of GDP, have been identified (Chardin  et al., 1996  ; Peyroche  et al., 1996  ; Klarlund  et al., 1997  ; Meacci  et al., 1997  ; Morinaga  et al., 1997  ; Sata  et al., 1998  ).	bind
50446	2	11546	6	NULL	NULL	0	NULL	GEF	NULL		promote	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_9_11_3133_s_37	9802902	A number of GEFs, which promote binding of GTP to ARF by facilitating the release of GDP, have been identified (Chardin  et al., 1996  ; Peyroche  et al., 1996  ; Klarlund  et al., 1997  ; Meacci  et al., 1997  ; Morinaga  et al., 1997  ; Sata  et al., 1998  ).	bind
50447	3	11546	6	NULL	NULL	0	NULL	GEF	NULL		facilitates	NULL				GDP	NULL	release of 			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_9_11_3133_s_37	9802902	A number of GEFs, which promote binding of GTP to ARF by facilitating the release of GDP, have been identified (Chardin  et al., 1996  ; Peyroche  et al., 1996  ; Klarlund  et al., 1997  ; Meacci  et al., 1997  ; Morinaga  et al., 1997  ; Sata  et al., 1998  ).	bind
50448	4	11546	6	NULL	NULL	0	NULL	statement 2	NULL		occurs via	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_9_11_3133_s_37	9802902	A number of GEFs, which promote binding of GTP to ARF by facilitating the release of GDP, have been identified (Chardin  et al., 1996  ; Peyroche  et al., 1996  ; Klarlund  et al., 1997  ; Meacci  et al., 1997  ; Morinaga  et al., 1997  ; Sata  et al., 1998  ).	bind
51113	1	11547	5	NULL	NULL	NULL	NULL	intimin	GP		bind		directly			host cells	Cell	uninfected			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_8_4637_s_189	10899867	A number of groups have reported that intimin can bind directly to uninfected host cells ( 2,  8) and to a receptor encoded by the bacteria, termed Tir, which is translocated into the host cell membrane via a type III secretion system ( 18).	bind
51114	2	11547	5	NULL	NULL	NULL	NULL	intimin	GP		bind		directly			Tir	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_8_4637_s_189	10899867	A number of groups have reported that intimin can bind directly to uninfected host cells ( 2,  8) and to a receptor encoded by the bacteria, termed Tir, which is translocated into the host cell membrane via a type III secretion system ( 18).	bind
51115	3	11547	5	NULL	NULL	NULL	NULL	Tir	GP		is a type of					receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_8_4637_s_189	10899867	A number of groups have reported that intimin can bind directly to uninfected host cells ( 2,  8) and to a receptor encoded by the bacteria, termed Tir, which is translocated into the host cell membrane via a type III secretion system ( 18).	bind
51116	4	11547	5	NULL	NULL	NULL	NULL	Tir	GP		is encoded by					bacteria	Organism				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_8_4637_s_189	10899867	A number of groups have reported that intimin can bind directly to uninfected host cells ( 2,  8) and to a receptor encoded by the bacteria, termed Tir, which is translocated into the host cell membrane via a type III secretion system ( 18).	bind
51117	5	11547	5	NULL	NULL	NULL	NULL	Tir	GP		is translocated to					host cell  membrane	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_8_4637_s_189	10899867	A number of groups have reported that intimin can bind directly to uninfected host cells ( 2,  8) and to a receptor encoded by the bacteria, termed Tir, which is translocated into the host cell membrane via a type III secretion system ( 18).	bind
51118	6	11547	5	NULL	NULL	NULL	NULL	statement 5	Process		via					type III secretion system	Process				NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_8_4637_s_189	10899867	A number of groups have reported that intimin can bind directly to uninfected host cells ( 2,  8) and to a receptor encoded by the bacteria, termed Tir, which is translocated into the host cell membrane via a type III secretion system ( 18).	bind
50449	1	11547	6	NULL	NULL	0	NULL	intimin	NULL		bind	NULL	directly			host cells	NULL	uninfected			NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_8_4637_s_189	10899867	A number of groups have reported that intimin can bind directly to uninfected host cells ( 2,  8) and to a receptor encoded by the bacteria, termed Tir, which is translocated into the host cell membrane via a type III secretion system ( 18).	bind
50450	2	11547	6	NULL	NULL	0	NULL	intimin	NULL		bind	NULL				Tir	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_8_4637_s_189	10899867	A number of groups have reported that intimin can bind directly to uninfected host cells ( 2,  8) and to a receptor encoded by the bacteria, termed Tir, which is translocated into the host cell membrane via a type III secretion system ( 18).	bind
50451	3	11547	6	10	NULL	0	NULL	Tir			is a type of					receptor  		bacteria			NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_8_4637_s_189	10899867	A number of groups have reported that intimin can bind directly to uninfected host cells ( 2,  8) and to a receptor encoded by the bacteria, termed Tir, which is translocated into the host cell membrane via a type III secretion system ( 18).	bind
50452	4	11547	6	NULL	NULL	0	NULL	Tir	NULL		is translocated into	NULL				host cell membrane	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_8_4637_s_189	10899867	A number of groups have reported that intimin can bind directly to uninfected host cells ( 2,  8) and to a receptor encoded by the bacteria, termed Tir, which is translocated into the host cell membrane via a type III secretion system ( 18).	bind
50453	5	11547	6	NULL	NULL	0	NULL	statement 4	NULL		occurs via	NULL				type III secretion system	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_8_4637_s_189	10899867	A number of groups have reported that intimin can bind directly to uninfected host cells ( 2,  8) and to a receptor encoded by the bacteria, termed Tir, which is translocated into the host cell membrane via a type III secretion system ( 18).	bind
51119	1	11548	5	NULL	NULL	NULL	NULL	GTP	Chemical		bind					Rho family members	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_52_33105_s_18	9407095	A number of guanine nucleotide exchange factors, which promote binding of GTP to Rho family members by facilitating the release of GDP, have been identified ( 16).	bind
51120	2	11548	5	NULL	NULL	NULL	NULL	guanine nucleotide exchange factors	GP		promotes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_52_33105_s_18	9407095	A number of guanine nucleotide exchange factors, which promote binding of GTP to Rho family members by facilitating the release of GDP, have been identified ( 16).	bind
51121	3	11548	5	NULL	NULL	NULL	NULL	guanine nucleotide exchange factors	GP		facilitates					GDP	Chemical	release of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_52_33105_s_18	9407095	A number of guanine nucleotide exchange factors, which promote binding of GTP to Rho family members by facilitating the release of GDP, have been identified ( 16).	bind
51122	4	11548	5	NULL	NULL	NULL	NULL	statement 3	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_52_33105_s_18	9407095	A number of guanine nucleotide exchange factors, which promote binding of GTP to Rho family members by facilitating the release of GDP, have been identified ( 16).	bind
50454	1	11548	6	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				Rho family members	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_52_33105_s_18	9407095	A number of guanine nucleotide exchange factors, which promote binding of GTP to Rho family members by facilitating the release of GDP, have been identified ( 16).	bind
50455	2	11548	6	NULL	NULL	0	NULL	guanine nucleotide exchange factors	NULL		promote	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_52_33105_s_18	9407095	A number of guanine nucleotide exchange factors, which promote binding of GTP to Rho family members by facilitating the release of GDP, have been identified ( 16).	bind
50456	3	11548	6	NULL	NULL	0	NULL	statement 2	NULL		occurs by facilitating	NULL				GDP	NULL	release of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_52_33105_s_18	9407095	A number of guanine nucleotide exchange factors, which promote binding of GTP to Rho family members by facilitating the release of GDP, have been identified ( 16).	bind
54192	4	11548	6	10	NULL	0	NULL	statement 3			leads to					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_52_33105_s_18	9407095	A number of guanine nucleotide exchange factors, which promote binding of GTP to Rho family members by facilitating the release of GDP, have been identified ( 16).	bind
51123	1	11549	5	NULL	NULL	NULL	NULL	HDAC	GP		is					histone deacetylases	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_131_24_6185_s_29	15548582	A number of histone deacetylases (HDAC) and histone methyltransferases (HMT) are associated with MeCP2, MBD1, MBD3 and DNA methyltransferases.	bind
51124	2	11549	5	NULL	NULL	NULL	NULL	HMT	GP		is					histone methyltransferases	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_131_24_6185_s_29	15548582	A number of histone deacetylases (HDAC) and histone methyltransferases (HMT) are associated with MeCP2, MBD1, MBD3 and DNA methyltransferases.	bind
51125	3	11549	5	NULL	NULL	NULL	NULL	HDAC	GP		is associated with					MeCP2	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_131_24_6185_s_29	15548582	A number of histone deacetylases (HDAC) and histone methyltransferases (HMT) are associated with MeCP2, MBD1, MBD3 and DNA methyltransferases.	bind
51126	4	11549	5	NULL	NULL	NULL	NULL	HDAC	GP		is associated with					MBD1	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_131_24_6185_s_29	15548582	A number of histone deacetylases (HDAC) and histone methyltransferases (HMT) are associated with MeCP2, MBD1, MBD3 and DNA methyltransferases.	bind
51127	5	11549	5	NULL	NULL	NULL	NULL	HDAC	GP		is associated with					MBD3	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_131_24_6185_s_29	15548582	A number of histone deacetylases (HDAC) and histone methyltransferases (HMT) are associated with MeCP2, MBD1, MBD3 and DNA methyltransferases.	bind
51128	6	11549	5	NULL	NULL	NULL	NULL	HDAC	GP		is associated with					DNA methyltransferases	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_131_24_6185_s_29	15548582	A number of histone deacetylases (HDAC) and histone methyltransferases (HMT) are associated with MeCP2, MBD1, MBD3 and DNA methyltransferases.	bind
51129	7	11549	5	NULL	NULL	NULL	NULL	HMT	GP		is associated with					MeCP2	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_131_24_6185_s_29	15548582	A number of histone deacetylases (HDAC) and histone methyltransferases (HMT) are associated with MeCP2, MBD1, MBD3 and DNA methyltransferases.	bind
51130	8	11549	5	NULL	NULL	NULL	NULL	HMT	GP		is associated with					MBD1	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_131_24_6185_s_29	15548582	A number of histone deacetylases (HDAC) and histone methyltransferases (HMT) are associated with MeCP2, MBD1, MBD3 and DNA methyltransferases.	bind
51131	9	11549	5	NULL	NULL	NULL	NULL	HMT	GP		is associated with					MBD3	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_131_24_6185_s_29	15548582	A number of histone deacetylases (HDAC) and histone methyltransferases (HMT) are associated with MeCP2, MBD1, MBD3 and DNA methyltransferases.	bind
51132	10	11549	5	NULL	NULL	NULL	NULL	HMT	GP		is associated with					DNA methyltransferases	GP				NULL		NULL	NULL	NULL	NULL	gw70_development_131_24_6185_s_29	15548582	A number of histone deacetylases (HDAC) and histone methyltransferases (HMT) are associated with MeCP2, MBD1, MBD3 and DNA methyltransferases.	bind
50469	1	11549	6	NULL	NULL	0	NULL	HDAC	NULL		is	NULL				histone deacetylase	NULL				NULL		0	NULL	NULL	NULL	gw70_development_131_24_6185_s_29	15548582	A number of histone deacetylases (HDAC) and histone methyltransferases (HMT) are associated with MeCP2, MBD1, MBD3 and DNA methyltransferases.	bind
50470	2	11549	6	NULL	NULL	0	NULL	HMT	NULL		is	NULL				histone methyltransferases	NULL				NULL		0	NULL	NULL	NULL	gw70_development_131_24_6185_s_29	15548582	A number of histone deacetylases (HDAC) and histone methyltransferases (HMT) are associated with MeCP2, MBD1, MBD3 and DNA methyltransferases.	bind
50471	3	11549	6	NULL	NULL	0	NULL	HDAC	NULL		associates with	NULL				MeCP2	NULL				NULL		0	NULL	NULL	NULL	gw70_development_131_24_6185_s_29	15548582	A number of histone deacetylases (HDAC) and histone methyltransferases (HMT) are associated with MeCP2, MBD1, MBD3 and DNA methyltransferases.	bind
50483	4	11549	6	NULL	NULL	0	NULL	HDAC	NULL		associates with	NULL				MBD1	NULL				NULL		0	NULL	NULL	NULL	gw70_development_131_24_6185_s_29	15548582	A number of histone deacetylases (HDAC) and histone methyltransferases (HMT) are associated with MeCP2, MBD1, MBD3 and DNA methyltransferases.	bind
50484	5	11549	6	NULL	NULL	0	NULL	HDAC	NULL		associates with	NULL				MBD3	NULL				NULL		0	NULL	NULL	NULL	gw70_development_131_24_6185_s_29	15548582	A number of histone deacetylases (HDAC) and histone methyltransferases (HMT) are associated with MeCP2, MBD1, MBD3 and DNA methyltransferases.	bind
50485	6	11549	6	NULL	NULL	0	NULL	HDAC	NULL		associates with	NULL				DNA methyltransferases	NULL				NULL		0	NULL	NULL	NULL	gw70_development_131_24_6185_s_29	15548582	A number of histone deacetylases (HDAC) and histone methyltransferases (HMT) are associated with MeCP2, MBD1, MBD3 and DNA methyltransferases.	bind
50486	7	11549	6	NULL	NULL	0	NULL	HMT	NULL		associates with	NULL				MeCP2	NULL				NULL		0	NULL	NULL	NULL	gw70_development_131_24_6185_s_29	15548582	A number of histone deacetylases (HDAC) and histone methyltransferases (HMT) are associated with MeCP2, MBD1, MBD3 and DNA methyltransferases.	bind
50487	8	11549	6	NULL	NULL	0	NULL	HMT	NULL		associates with	NULL				MBD1	NULL				NULL		0	NULL	NULL	NULL	gw70_development_131_24_6185_s_29	15548582	A number of histone deacetylases (HDAC) and histone methyltransferases (HMT) are associated with MeCP2, MBD1, MBD3 and DNA methyltransferases.	bind
50488	9	11549	6	NULL	NULL	0	NULL	HMT	NULL		associates with	NULL				MBD3	NULL				NULL		0	NULL	NULL	NULL	gw70_development_131_24_6185_s_29	15548582	A number of histone deacetylases (HDAC) and histone methyltransferases (HMT) are associated with MeCP2, MBD1, MBD3 and DNA methyltransferases.	bind
50489	10	11549	6	NULL	NULL	0	NULL	HMT	NULL		associates with	NULL				DNA methyltransferases	NULL				NULL		0	NULL	NULL	NULL	gw70_development_131_24_6185_s_29	15548582	A number of histone deacetylases (HDAC) and histone methyltransferases (HMT) are associated with MeCP2, MBD1, MBD3 and DNA methyltransferases.	bind
51133	1	11550	5	NULL	NULL	NULL	NULL	FK506	Chemical		is a type of					immunosuppressant	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_14_8351_s_187	9653190	A number of immunophilin ligands, including the immunosuppressant FK506, which also binds to FKBP12, are neurotrophic ( 22).	bind
51134	2	11550	5	NULL	NULL	NULL	NULL	FK506	Chemical		is a type of					immunophilin ligand	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_14_8351_s_187	9653190	A number of immunophilin ligands, including the immunosuppressant FK506, which also binds to FKBP12, are neurotrophic ( 22).	bind
51135	3	11550	5	NULL	NULL	NULL	NULL	FK506	Chemical		bind					FKBP12	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_14_8351_s_187	9653190	A number of immunophilin ligands, including the immunosuppressant FK506, which also binds to FKBP12, are neurotrophic ( 22).	bind
50490	1	11550	6	10	NULL	0	NULL	FK506			bind					FKBP12					NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_14_8351_s_187	9653190	A number of immunophilin ligands, including the immunosuppressant FK506, which also binds to FKBP12, are neurotrophic ( 22).	bind
50491	2	11550	6	NULL	NULL	0	NULL	FK506	NULL		is a type of	NULL				immunophilin ligand	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_14_8351_s_187	9653190	A number of immunophilin ligands, including the immunosuppressant FK506, which also binds to FKBP12, are neurotrophic ( 22).	bind
50492	3	11550	6	NULL	NULL	0	NULL	FKBP12	NULL		is	NULL				neurotrophic	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_95_14_8351_s_187	9653190	A number of immunophilin ligands, including the immunosuppressant FK506, which also binds to FKBP12, are neurotrophic ( 22).	bind
54193	4	11550	6	10	NULL	0	NULL	FK506			is a type of					immunosuppressant					NULL		0	NULL	NULL	NULL	gw60_pnas_95_14_8351_s_187	9653190	A number of immunophilin ligands, including the immunosuppressant FK506, which also binds to FKBP12, are neurotrophic ( 22).	bind
51136	1	11551	5	NULL	NULL	NULL	NULL	Tau	GP		bind					MTs	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_39_30335_s_20	10869348	A number of investigations on the binding of Tau to MTs have been reported ( 6-14).	bind
50493	1	11551	6	NULL	NULL	0	NULL	Tau	NULL		bind	NULL				MTs	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_39_30335_s_20	10869348	A number of investigations on the binding of Tau to MTs have been reported ( 6-14).	bind
51137	1	11552	5	NULL	NULL	NULL	NULL	KAP-1	GP		mediates							repression of	KRAB domain		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4366_s_30	10330177	A number of lines of evidence have suggested that KAP-1 plays a key role in mediating KRAB domain repression: (i) KAP-1 binds to multiple KRAB repression domains both in vitro and in vivo, (ii) KRAB domain mutations which abolish repression decrease or eliminate the interaction with KAP-1, (iii) overexpression of KAP-1 enhances KRAB-mediated repression in a manner dependent on the presence of the RBCC domain, and (iv) heterologous fusions between KAP-1 and a DNA binding domain can potentiate repression ( 17,  36,  42).	bind
51138	2	11552	5	NULL	NULL	NULL	NULL	KAP-1	GP		bind							multiple	KRAB repression domains		NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4366_s_30	10330177	A number of lines of evidence have suggested that KAP-1 plays a key role in mediating KRAB domain repression: (i) KAP-1 binds to multiple KRAB repression domains both in vitro and in vivo, (ii) KRAB domain mutations which abolish repression decrease or eliminate the interaction with KAP-1, (iii) overexpression of KAP-1 enhances KRAB-mediated repression in a manner dependent on the presence of the RBCC domain, and (iv) heterologous fusions between KAP-1 and a DNA binding domain can potentiate repression ( 17,  36,  42).	bind
51139	3	11552	5	NULL	NULL	NULL	NULL	KAP-1	GP		bind							multiple	KRAB repression domains		NULL	in vivo	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4366_s_30	10330177	A number of lines of evidence have suggested that KAP-1 plays a key role in mediating KRAB domain repression: (i) KAP-1 binds to multiple KRAB repression domains both in vitro and in vivo, (ii) KRAB domain mutations which abolish repression decrease or eliminate the interaction with KAP-1, (iii) overexpression of KAP-1 enhances KRAB-mediated repression in a manner dependent on the presence of the RBCC domain, and (iv) heterologous fusions between KAP-1 and a DNA binding domain can potentiate repression ( 17,  36,  42).	bind
51140	4	11552	5	NULL	NULL	NULL	NULL			mutant	abolishes			KRAB domain		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4366_s_30	10330177	A number of lines of evidence have suggested that KAP-1 plays a key role in mediating KRAB domain repression: (i) KAP-1 binds to multiple KRAB repression domains both in vitro and in vivo, (ii) KRAB domain mutations which abolish repression decrease or eliminate the interaction with KAP-1, (iii) overexpression of KAP-1 enhances KRAB-mediated repression in a manner dependent on the presence of the RBCC domain, and (iv) heterologous fusions between KAP-1 and a DNA binding domain can potentiate repression ( 17,  36,  42).	bind
51141	5	11552	5	NULL	NULL	NULL	NULL			mutant	abolishes			KRAB domain		repression	Process	decrease of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4366_s_30	10330177	A number of lines of evidence have suggested that KAP-1 plays a key role in mediating KRAB domain repression: (i) KAP-1 binds to multiple KRAB repression domains both in vitro and in vivo, (ii) KRAB domain mutations which abolish repression decrease or eliminate the interaction with KAP-1, (iii) overexpression of KAP-1 enhances KRAB-mediated repression in a manner dependent on the presence of the RBCC domain, and (iv) heterologous fusions between KAP-1 and a DNA binding domain can potentiate repression ( 17,  36,  42).	bind
51143	6	11552	5	NULL	NULL	NULL	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4366_s_30	10330177	A number of lines of evidence have suggested that KAP-1 plays a key role in mediating KRAB domain repression: (i) KAP-1 binds to multiple KRAB repression domains both in vitro and in vivo, (ii) KRAB domain mutations which abolish repression decrease or eliminate the interaction with KAP-1, (iii) overexpression of KAP-1 enhances KRAB-mediated repression in a manner dependent on the presence of the RBCC domain, and (iv) heterologous fusions between KAP-1 and a DNA binding domain can potentiate repression ( 17,  36,  42).	bind
51144	7	11552	5	NULL	NULL	NULL	NULL	KAP-1	GP	overexpression of	enhances					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4366_s_30	10330177	A number of lines of evidence have suggested that KAP-1 plays a key role in mediating KRAB domain repression: (i) KAP-1 binds to multiple KRAB repression domains both in vitro and in vivo, (ii) KRAB domain mutations which abolish repression decrease or eliminate the interaction with KAP-1, (iii) overexpression of KAP-1 enhances KRAB-mediated repression in a manner dependent on the presence of the RBCC domain, and (iv) heterologous fusions between KAP-1 and a DNA binding domain can potentiate repression ( 17,  36,  42).	bind
51145	8	11552	5	NULL	NULL	NULL	NULL	statement 7	Process		is dependent on							presence of	RBCC domain		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4366_s_30	10330177	A number of lines of evidence have suggested that KAP-1 plays a key role in mediating KRAB domain repression: (i) KAP-1 binds to multiple KRAB repression domains both in vitro and in vivo, (ii) KRAB domain mutations which abolish repression decrease or eliminate the interaction with KAP-1, (iii) overexpression of KAP-1 enhances KRAB-mediated repression in a manner dependent on the presence of the RBCC domain, and (iv) heterologous fusions between KAP-1 and a DNA binding domain can potentiate repression ( 17,  36,  42).	bind
51146	9	11552	5	NULL	NULL	NULL	NULL	KAP-1	GP		is fused to		heterologous						DNA binding domain		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4366_s_30	10330177	A number of lines of evidence have suggested that KAP-1 plays a key role in mediating KRAB domain repression: (i) KAP-1 binds to multiple KRAB repression domains both in vitro and in vivo, (ii) KRAB domain mutations which abolish repression decrease or eliminate the interaction with KAP-1, (iii) overexpression of KAP-1 enhances KRAB-mediated repression in a manner dependent on the presence of the RBCC domain, and (iv) heterologous fusions between KAP-1 and a DNA binding domain can potentiate repression ( 17,  36,  42).	bind
51147	10	11552	5	NULL	NULL	NULL	NULL	statement 9	Process		potentiate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4366_s_30	10330177	A number of lines of evidence have suggested that KAP-1 plays a key role in mediating KRAB domain repression: (i) KAP-1 binds to multiple KRAB repression domains both in vitro and in vivo, (ii) KRAB domain mutations which abolish repression decrease or eliminate the interaction with KAP-1, (iii) overexpression of KAP-1 enhances KRAB-mediated repression in a manner dependent on the presence of the RBCC domain, and (iv) heterologous fusions between KAP-1 and a DNA binding domain can potentiate repression ( 17,  36,  42).	bind
50494	1	11552	6	10	NULL	0	NULL	KAP-1			mediates							repression of	KRAB domain		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4366_s_30	10330177	A number of lines of evidence have suggested that KAP-1 plays a key role in mediating KRAB domain repression: (i) KAP-1 binds to multiple KRAB repression domains both in vitro and in vivo, (ii) KRAB domain mutations which abolish repression decrease or eliminate the interaction with KAP-1, (iii) overexpression of KAP-1 enhances KRAB-mediated repression in a manner dependent on the presence of the RBCC domain, and (iv) heterologous fusions between KAP-1 and a DNA binding domain can potentiate repression ( 17,  36,  42).	bind
50495	2	11552	6	NULL	NULL	0	NULL	KAP-1	NULL		bind	NULL					NULL		KRAB repression domain		NULL	in vitro	0	NULL	NULL	NULL	gw60_molcellbiol_19_6_4366_s_30	10330177	A number of lines of evidence have suggested that KAP-1 plays a key role in mediating KRAB domain repression: (i) KAP-1 binds to multiple KRAB repression domains both in vitro and in vivo, (ii) KRAB domain mutations which abolish repression decrease or eliminate the interaction with KAP-1, (iii) overexpression of KAP-1 enhances KRAB-mediated repression in a manner dependent on the presence of the RBCC domain, and (iv) heterologous fusions between KAP-1 and a DNA binding domain can potentiate repression ( 17,  36,  42).	bind
50496	3	11552	6	NULL	NULL	0	NULL	KAP-1	NULL		bind	NULL					NULL		KRAB repression domain		NULL	in vivo	0	NULL	NULL	NULL	gw60_molcellbiol_19_6_4366_s_30	10330177	A number of lines of evidence have suggested that KAP-1 plays a key role in mediating KRAB domain repression: (i) KAP-1 binds to multiple KRAB repression domains both in vitro and in vivo, (ii) KRAB domain mutations which abolish repression decrease or eliminate the interaction with KAP-1, (iii) overexpression of KAP-1 enhances KRAB-mediated repression in a manner dependent on the presence of the RBCC domain, and (iv) heterologous fusions between KAP-1 and a DNA binding domain can potentiate repression ( 17,  36,  42).	bind
50538	4	11552	6	NULL	NULL	0	NULL		NULL	mutation of	eliminates	NULL		KRAB domain		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_6_4366_s_30	10330177	A number of lines of evidence have suggested that KAP-1 plays a key role in mediating KRAB domain repression: (i) KAP-1 binds to multiple KRAB repression domains both in vitro and in vivo, (ii) KRAB domain mutations which abolish repression decrease or eliminate the interaction with KAP-1, (iii) overexpression of KAP-1 enhances KRAB-mediated repression in a manner dependent on the presence of the RBCC domain, and (iv) heterologous fusions between KAP-1 and a DNA binding domain can potentiate repression ( 17,  36,  42).	bind
50539	5	11552	6	10	NULL	0	NULL			mutant	abolishes			KRAB domain		repression		decrease of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4366_s_30	10330177	A number of lines of evidence have suggested that KAP-1 plays a key role in mediating KRAB domain repression: (i) KAP-1 binds to multiple KRAB repression domains both in vitro and in vivo, (ii) KRAB domain mutations which abolish repression decrease or eliminate the interaction with KAP-1, (iii) overexpression of KAP-1 enhances KRAB-mediated repression in a manner dependent on the presence of the RBCC domain, and (iv) heterologous fusions between KAP-1 and a DNA binding domain can potentiate repression ( 17,  36,  42).	bind
50540	6	11552	6	10	NULL	0	NULL	KAP-1		overexpression of	enhances					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_6_4366_s_30	10330177	A number of lines of evidence have suggested that KAP-1 plays a key role in mediating KRAB domain repression: (i) KAP-1 binds to multiple KRAB repression domains both in vitro and in vivo, (ii) KRAB domain mutations which abolish repression decrease or eliminate the interaction with KAP-1, (iii) overexpression of KAP-1 enhances KRAB-mediated repression in a manner dependent on the presence of the RBCC domain, and (iv) heterologous fusions between KAP-1 and a DNA binding domain can potentiate repression ( 17,  36,  42).	bind
50541	7	11552	6	NULL	NULL	0	NULL	statement 6	NULL		is dependent on	NULL					NULL	presence of	RBCC domain		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_6_4366_s_30	10330177	A number of lines of evidence have suggested that KAP-1 plays a key role in mediating KRAB domain repression: (i) KAP-1 binds to multiple KRAB repression domains both in vitro and in vivo, (ii) KRAB domain mutations which abolish repression decrease or eliminate the interaction with KAP-1, (iii) overexpression of KAP-1 enhances KRAB-mediated repression in a manner dependent on the presence of the RBCC domain, and (iv) heterologous fusions between KAP-1 and a DNA binding domain can potentiate repression ( 17,  36,  42).	bind
50542	8	11552	6	NULL	NULL	0	NULL	KAP-1	NULL		fuses with	NULL					NULL		DNA binding domain		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_6_4366_s_30	10330177	A number of lines of evidence have suggested that KAP-1 plays a key role in mediating KRAB domain repression: (i) KAP-1 binds to multiple KRAB repression domains both in vitro and in vivo, (ii) KRAB domain mutations which abolish repression decrease or eliminate the interaction with KAP-1, (iii) overexpression of KAP-1 enhances KRAB-mediated repression in a manner dependent on the presence of the RBCC domain, and (iv) heterologous fusions between KAP-1 and a DNA binding domain can potentiate repression ( 17,  36,  42).	bind
50543	9	11552	6	NULL	NULL	0	NULL	statement 8	NULL		potentiate	NULL				repression	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_6_4366_s_30	10330177	A number of lines of evidence have suggested that KAP-1 plays a key role in mediating KRAB domain repression: (i) KAP-1 binds to multiple KRAB repression domains both in vitro and in vivo, (ii) KRAB domain mutations which abolish repression decrease or eliminate the interaction with KAP-1, (iii) overexpression of KAP-1 enhances KRAB-mediated repression in a manner dependent on the presence of the RBCC domain, and (iv) heterologous fusions between KAP-1 and a DNA binding domain can potentiate repression ( 17,  36,  42).	bind
54195	10	11552	6	10	NULL	0	NULL	statement 4			is an alternative to					statement 5					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_6_4366_s_30	10330177	A number of lines of evidence have suggested that KAP-1 plays a key role in mediating KRAB domain repression: (i) KAP-1 binds to multiple KRAB repression domains both in vitro and in vivo, (ii) KRAB domain mutations which abolish repression decrease or eliminate the interaction with KAP-1, (iii) overexpression of KAP-1 enhances KRAB-mediated repression in a manner dependent on the presence of the RBCC domain, and (iv) heterologous fusions between KAP-1 and a DNA binding domain can potentiate repression ( 17,  36,  42).	bind
51148	1	11553	5	NULL	NULL	NULL	NULL	VnbP	GP		bind					vitronectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclinmicrobiol_38_1_389_s_90	10618121	A number of matrix binding proteins have been described for GAS, including SfbI ( 25), SfbII ( 15), F1 ( 10) and FBBP ( 4) (which each bind to fibronectin), and VnbP, which binds to vitronectin ( 17).	bind
51149	2	11553	5	NULL	NULL	NULL	NULL	SfbI	GP		bind					fibronectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclinmicrobiol_38_1_389_s_90	10618121	A number of matrix binding proteins have been described for GAS, including SfbI ( 25), SfbII ( 15), F1 ( 10) and FBBP ( 4) (which each bind to fibronectin), and VnbP, which binds to vitronectin ( 17).	bind
51150	3	11553	5	NULL	NULL	NULL	NULL	SfbII	GP		bind					fibronectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclinmicrobiol_38_1_389_s_90	10618121	A number of matrix binding proteins have been described for GAS, including SfbI ( 25), SfbII ( 15), F1 ( 10) and FBBP ( 4) (which each bind to fibronectin), and VnbP, which binds to vitronectin ( 17).	bind
51151	4	11553	5	NULL	NULL	NULL	NULL	F1	GP		bind					fibronectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclinmicrobiol_38_1_389_s_90	10618121	A number of matrix binding proteins have been described for GAS, including SfbI ( 25), SfbII ( 15), F1 ( 10) and FBBP ( 4) (which each bind to fibronectin), and VnbP, which binds to vitronectin ( 17).	bind
51152	5	11553	5	NULL	NULL	NULL	NULL	FBBP	GP		bind					fibronectin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jclinmicrobiol_38_1_389_s_90	10618121	A number of matrix binding proteins have been described for GAS, including SfbI ( 25), SfbII ( 15), F1 ( 10) and FBBP ( 4) (which each bind to fibronectin), and VnbP, which binds to vitronectin ( 17).	bind
50544	1	11553	6	NULL	NULL	0	NULL	SfbI	NULL		bind	NULL				fibronectin	NULL				NULL		0	NULL	NULL	NULL	gw60_jclinmicrobiol_38_1_389_s_90	10618121	A number of matrix binding proteins have been described for GAS, including SfbI ( 25), SfbII ( 15), F1 ( 10) and FBBP ( 4) (which each bind to fibronectin), and VnbP, which binds to vitronectin ( 17).	bind
50545	2	11553	6	NULL	NULL	0	NULL	SfbII	NULL		bind	NULL				fibronectin	NULL				NULL		0	NULL	NULL	NULL	gw60_jclinmicrobiol_38_1_389_s_90	10618121	A number of matrix binding proteins have been described for GAS, including SfbI ( 25), SfbII ( 15), F1 ( 10) and FBBP ( 4) (which each bind to fibronectin), and VnbP, which binds to vitronectin ( 17).	bind
50546	3	11553	6	NULL	NULL	0	NULL	F1	NULL		bind	NULL				fibronectin	NULL				NULL		0	NULL	NULL	NULL	gw60_jclinmicrobiol_38_1_389_s_90	10618121	A number of matrix binding proteins have been described for GAS, including SfbI ( 25), SfbII ( 15), F1 ( 10) and FBBP ( 4) (which each bind to fibronectin), and VnbP, which binds to vitronectin ( 17).	bind
50547	4	11553	6	NULL	NULL	0	NULL	FBBP	NULL		bind	NULL				fibronectin	NULL				NULL		0	NULL	NULL	NULL	gw60_jclinmicrobiol_38_1_389_s_90	10618121	A number of matrix binding proteins have been described for GAS, including SfbI ( 25), SfbII ( 15), F1 ( 10) and FBBP ( 4) (which each bind to fibronectin), and VnbP, which binds to vitronectin ( 17).	bind
50548	5	11553	6	NULL	NULL	0	NULL	VnbP	NULL		bind	NULL				vitronectin	NULL				NULL		0	NULL	NULL	NULL	gw60_jclinmicrobiol_38_1_389_s_90	10618121	A number of matrix binding proteins have been described for GAS, including SfbI ( 25), SfbII ( 15), F1 ( 10) and FBBP ( 4) (which each bind to fibronectin), and VnbP, which binds to vitronectin ( 17).	bind
51153	1	11554	5	NULL	NULL	NULL	NULL	ERK	GP		phosphorylates					SOS	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_9_2863_s_322	10982386	A number of mechanisms have been proposed to be involved in this down-regulation of the pathway, including ERK phosphorylation of SOS, which prevents SOS binding to Grb2 (Langlois  et al., 1995  ; Corbalan-Garcia  et al., 1996  ).	bind
51154	2	11554	5	NULL	NULL	NULL	NULL	SOS	GP		bind					Grb2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_9_2863_s_322	10982386	A number of mechanisms have been proposed to be involved in this down-regulation of the pathway, including ERK phosphorylation of SOS, which prevents SOS binding to Grb2 (Langlois  et al., 1995  ; Corbalan-Garcia  et al., 1996  ).	bind
51155	3	11554	5	NULL	NULL	NULL	NULL	statement 1	Process		prevents					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_9_2863_s_322	10982386	A number of mechanisms have been proposed to be involved in this down-regulation of the pathway, including ERK phosphorylation of SOS, which prevents SOS binding to Grb2 (Langlois  et al., 1995  ; Corbalan-Garcia  et al., 1996  ).	bind
50549	1	11554	6	NULL	NULL	0	NULL	SOS	NULL		bind	NULL				Grb2	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_9_2863_s_322	10982386	A number of mechanisms have been proposed to be involved in this down-regulation of the pathway, including ERK phosphorylation of SOS, which prevents SOS binding to Grb2 (Langlois  et al., 1995  ; Corbalan-Garcia  et al., 1996  ).	bind
50550	2	11554	6	NULL	NULL	0	NULL	ERK	NULL		phosphorylates	NULL				SOS	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_9_2863_s_322	10982386	A number of mechanisms have been proposed to be involved in this down-regulation of the pathway, including ERK phosphorylation of SOS, which prevents SOS binding to Grb2 (Langlois  et al., 1995  ; Corbalan-Garcia  et al., 1996  ).	bind
50551	3	11554	6	NULL	NULL	0	NULL	statement 2	NULL		prevents	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_9_2863_s_322	10982386	A number of mechanisms have been proposed to be involved in this down-regulation of the pathway, including ERK phosphorylation of SOS, which prevents SOS binding to Grb2 (Langlois  et al., 1995  ; Corbalan-Garcia  et al., 1996  ).	bind
51156	1	11555	5	NULL	NULL	NULL	NULL	SRF	GP		bind									CArG elements	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_14_8398_s_24	9525950	A number of mechanisms have been shown to increase SRF binding to CArG elements including post-translational modification of SRF ( 17), increased SRF protein expression ( 34), and interaction of SRF with homeodomain factors that modulate SRF binding or kinetics ( 38).	bind
51157	2	11555	5	NULL	NULL	NULL	NULL	SRF	GP	post-translational modification of	increases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_14_8398_s_24	9525950	A number of mechanisms have been shown to increase SRF binding to CArG elements including post-translational modification of SRF ( 17), increased SRF protein expression ( 34), and interaction of SRF with homeodomain factors that modulate SRF binding or kinetics ( 38).	bind
51158	3	11555	5	NULL	NULL	NULL	NULL	SRF protein	GP	increased expression of	increases					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_14_8398_s_24	9525950	A number of mechanisms have been shown to increase SRF binding to CArG elements including post-translational modification of SRF ( 17), increased SRF protein expression ( 34), and interaction of SRF with homeodomain factors that modulate SRF binding or kinetics ( 38).	bind
51159	4	11555	5	NULL	NULL	NULL	NULL	SRF	GP		interacts with					homeodomain factors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_14_8398_s_24	9525950	A number of mechanisms have been shown to increase SRF binding to CArG elements including post-translational modification of SRF ( 17), increased SRF protein expression ( 34), and interaction of SRF with homeodomain factors that modulate SRF binding or kinetics ( 38).	bind
51160	5	11555	5	NULL	NULL	NULL	NULL	statement 4	Process		modulates					SRF	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_14_8398_s_24	9525950	A number of mechanisms have been shown to increase SRF binding to CArG elements including post-translational modification of SRF ( 17), increased SRF protein expression ( 34), and interaction of SRF with homeodomain factors that modulate SRF binding or kinetics ( 38).	bind
50552	1	11555	6	NULL	NULL	0	NULL	SRF	NULL		bind	NULL					NULL			CArG element	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8398_s_24	9525950	A number of mechanisms have been shown to increase SRF binding to CArG elements including post-translational modification of SRF ( 17), increased SRF protein expression ( 34), and interaction of SRF with homeodomain factors that modulate SRF binding or kinetics ( 38).	bind
50553	2	11555	6	NULL	NULL	0	NULL	SRF	NULL	post-translational modification of	increase	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_14_8398_s_24	9525950	A number of mechanisms have been shown to increase SRF binding to CArG elements including post-translational modification of SRF ( 17), increased SRF protein expression ( 34), and interaction of SRF with homeodomain factors that modulate SRF binding or kinetics ( 38).	bind
50555	3	11555	6	NULL	NULL	0	NULL	SRF	NULL		interacts with	NULL				homeodomain factors	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8398_s_24	9525950	A number of mechanisms have been shown to increase SRF binding to CArG elements including post-translational modification of SRF ( 17), increased SRF protein expression ( 34), and interaction of SRF with homeodomain factors that modulate SRF binding or kinetics ( 38).	bind
54196	4	11555	6	10	NULL	0	NULL	statement 3			modulate					SRF		binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8398_s_24	9525950	A number of mechanisms have been shown to increase SRF binding to CArG elements including post-translational modification of SRF ( 17), increased SRF protein expression ( 34), and interaction of SRF with homeodomain factors that modulate SRF binding or kinetics ( 38).	bind
54197	5	11555	6	10	NULL	0	NULL	SRF		increased expression of	increase					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_14_8398_s_24	9525950	A number of mechanisms have been shown to increase SRF binding to CArG elements including post-translational modification of SRF ( 17), increased SRF protein expression ( 34), and interaction of SRF with homeodomain factors that modulate SRF binding or kinetics ( 38).	bind
51161	1	11556	5	NULL	NULL	NULL	NULL	cytochrome c	GP		bind					CcP	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1597_2_193_s_309	12044899	A number of models can be applied to the binding of cytochrome  c to CcP, ranging from a unique-independent sites model to a multiple-interacting sites model.	bind
50497	1	11556	6	NULL	NULL	0	NULL	cytochrome c	NULL		bind	NULL				CcP	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1597_2_193_s_309	12044899	A number of models can be applied to the binding of cytochrome  c to CcP, ranging from a unique-independent sites model to a multiple-interacting sites model.	bind
51162	1	11557	5	NULL	NULL	NULL	NULL	Munc18/n-Sec1/rbSec1	GP		bind					SNARE proteins	GP	individual			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_24_14038_s_14	11707603	A number of molecules (including Munc18/n-Sec1/rbSec1, complexins, Munc-13, tomosyn, snapin, and syntaphilin that bind to individual SNARE proteins) have been suggested to regulate the availability and/or propensity of free SNARE proteins to form functional release machinery ( 19-25).	bind
51163	2	11557	5	NULL	NULL	NULL	NULL	complexins	GP		bind					SNARE proteins	GP	individual			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_24_14038_s_14	11707603	A number of molecules (including Munc18/n-Sec1/rbSec1, complexins, Munc-13, tomosyn, snapin, and syntaphilin that bind to individual SNARE proteins) have been suggested to regulate the availability and/or propensity of free SNARE proteins to form functional release machinery ( 19-25).	bind
51164	3	11557	5	NULL	NULL	NULL	NULL	Munc-13	GP		bind					SNARE proteins	GP	individual			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_24_14038_s_14	11707603	A number of molecules (including Munc18/n-Sec1/rbSec1, complexins, Munc-13, tomosyn, snapin, and syntaphilin that bind to individual SNARE proteins) have been suggested to regulate the availability and/or propensity of free SNARE proteins to form functional release machinery ( 19-25).	bind
51165	4	11557	5	NULL	NULL	NULL	NULL	tomosyn	GP		bind					SNARE proteins	GP	individual			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_24_14038_s_14	11707603	A number of molecules (including Munc18/n-Sec1/rbSec1, complexins, Munc-13, tomosyn, snapin, and syntaphilin that bind to individual SNARE proteins) have been suggested to regulate the availability and/or propensity of free SNARE proteins to form functional release machinery ( 19-25).	bind
51166	5	11557	5	NULL	NULL	NULL	NULL	snapin	GP		bind					SNARE proteins	GP	individual			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_24_14038_s_14	11707603	A number of molecules (including Munc18/n-Sec1/rbSec1, complexins, Munc-13, tomosyn, snapin, and syntaphilin that bind to individual SNARE proteins) have been suggested to regulate the availability and/or propensity of free SNARE proteins to form functional release machinery ( 19-25).	bind
51167	6	11557	5	NULL	NULL	NULL	NULL	syntaphilin	GP		bind					SNARE proteins	GP	individual			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_24_14038_s_14	11707603	A number of molecules (including Munc18/n-Sec1/rbSec1, complexins, Munc-13, tomosyn, snapin, and syntaphilin that bind to individual SNARE proteins) have been suggested to regulate the availability and/or propensity of free SNARE proteins to form functional release machinery ( 19-25).	bind
51168	7	11557	5	NULL	NULL	NULL	NULL	SNARE proteins	GP	free	forms					functional release machinery	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_24_14038_s_14	11707603	A number of molecules (including Munc18/n-Sec1/rbSec1, complexins, Munc-13, tomosyn, snapin, and syntaphilin that bind to individual SNARE proteins) have been suggested to regulate the availability and/or propensity of free SNARE proteins to form functional release machinery ( 19-25).	bind
51169	8	11557	5	NULL	NULL	NULL	NULL	Munc18/n-Sec1/rbSec1	GP		regulates					statement 7	Process	availability;;propensity of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_24_14038_s_14	11707603	A number of molecules (including Munc18/n-Sec1/rbSec1, complexins, Munc-13, tomosyn, snapin, and syntaphilin that bind to individual SNARE proteins) have been suggested to regulate the availability and/or propensity of free SNARE proteins to form functional release machinery ( 19-25).	bind
51170	9	11557	5	NULL	NULL	NULL	NULL	complexins	GP		regulates					statement 7	Process	availability;;propensity of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_24_14038_s_14	11707603	A number of molecules (including Munc18/n-Sec1/rbSec1, complexins, Munc-13, tomosyn, snapin, and syntaphilin that bind to individual SNARE proteins) have been suggested to regulate the availability and/or propensity of free SNARE proteins to form functional release machinery ( 19-25).	bind
51171	10	11557	5	NULL	NULL	NULL	NULL	Munc-13	GP		regulates					statement 7	Process	availability;;propensity of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_24_14038_s_14	11707603	A number of molecules (including Munc18/n-Sec1/rbSec1, complexins, Munc-13, tomosyn, snapin, and syntaphilin that bind to individual SNARE proteins) have been suggested to regulate the availability and/or propensity of free SNARE proteins to form functional release machinery ( 19-25).	bind
51172	11	11557	5	NULL	NULL	NULL	NULL	tomosyn	GP		regulates					statement 7	Process	availability;;propensity of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_24_14038_s_14	11707603	A number of molecules (including Munc18/n-Sec1/rbSec1, complexins, Munc-13, tomosyn, snapin, and syntaphilin that bind to individual SNARE proteins) have been suggested to regulate the availability and/or propensity of free SNARE proteins to form functional release machinery ( 19-25).	bind
51173	12	11557	5	NULL	NULL	NULL	NULL	snapin	GP		regulates					statement 7	Process	availability;;propensity of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_24_14038_s_14	11707603	A number of molecules (including Munc18/n-Sec1/rbSec1, complexins, Munc-13, tomosyn, snapin, and syntaphilin that bind to individual SNARE proteins) have been suggested to regulate the availability and/or propensity of free SNARE proteins to form functional release machinery ( 19-25).	bind
51174	13	11557	5	NULL	NULL	NULL	NULL	syntaphilin	GP		regulates					statement 7	Process	availability;;propensity of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_24_14038_s_14	11707603	A number of molecules (including Munc18/n-Sec1/rbSec1, complexins, Munc-13, tomosyn, snapin, and syntaphilin that bind to individual SNARE proteins) have been suggested to regulate the availability and/or propensity of free SNARE proteins to form functional release machinery ( 19-25).	bind
50498	1	11557	6	NULL	NULL	0	NULL	Munc18/n-Sec1/rbSec1	NULL		bind	NULL				SNARE protein	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_98_24_14038_s_14	11707603	A number of molecules (including Munc18/n-Sec1/rbSec1, complexins, Munc-13, tomosyn, snapin, and syntaphilin that bind to individual SNARE proteins) have been suggested to regulate the availability and/or propensity of free SNARE proteins to form functional release machinery ( 19-25).	bind
50499	2	11557	6	NULL	NULL	0	NULL	complexins	NULL		bind	NULL				SNARE protein	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_98_24_14038_s_14	11707603	A number of molecules (including Munc18/n-Sec1/rbSec1, complexins, Munc-13, tomosyn, snapin, and syntaphilin that bind to individual SNARE proteins) have been suggested to regulate the availability and/or propensity of free SNARE proteins to form functional release machinery ( 19-25).	bind
50500	3	11557	6	NULL	NULL	0	NULL	Munc-13	NULL		bind	NULL				SNARE protein	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_98_24_14038_s_14	11707603	A number of molecules (including Munc18/n-Sec1/rbSec1, complexins, Munc-13, tomosyn, snapin, and syntaphilin that bind to individual SNARE proteins) have been suggested to regulate the availability and/or propensity of free SNARE proteins to form functional release machinery ( 19-25).	bind
50501	4	11557	6	NULL	NULL	0	NULL	tomosyn	NULL		bind	NULL				SNARE protein	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_98_24_14038_s_14	11707603	A number of molecules (including Munc18/n-Sec1/rbSec1, complexins, Munc-13, tomosyn, snapin, and syntaphilin that bind to individual SNARE proteins) have been suggested to regulate the availability and/or propensity of free SNARE proteins to form functional release machinery ( 19-25).	bind
50556	5	11557	6	NULL	NULL	0	NULL	snapin	NULL		bind	NULL				SNARE protein	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_98_24_14038_s_14	11707603	A number of molecules (including Munc18/n-Sec1/rbSec1, complexins, Munc-13, tomosyn, snapin, and syntaphilin that bind to individual SNARE proteins) have been suggested to regulate the availability and/or propensity of free SNARE proteins to form functional release machinery ( 19-25).	bind
50557	6	11557	6	NULL	NULL	0	NULL	syntaphilin	NULL		bind	NULL				SNARE protein	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_98_24_14038_s_14	11707603	A number of molecules (including Munc18/n-Sec1/rbSec1, complexins, Munc-13, tomosyn, snapin, and syntaphilin that bind to individual SNARE proteins) have been suggested to regulate the availability and/or propensity of free SNARE proteins to form functional release machinery ( 19-25).	bind
50558	7	11557	6	10	NULL	0	NULL	SNARE protein		free	forms					functional release machinery					NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_24_14038_s_14	11707603	A number of molecules (including Munc18/n-Sec1/rbSec1, complexins, Munc-13, tomosyn, snapin, and syntaphilin that bind to individual SNARE proteins) have been suggested to regulate the availability and/or propensity of free SNARE proteins to form functional release machinery ( 19-25).	bind
50559	8	11557	6	10	NULL	0	NULL	Munc18/n-Sec1/rbSec1			regulates					statement 7		availability of;;propensity of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_24_14038_s_14	11707603	A number of molecules (including Munc18/n-Sec1/rbSec1, complexins, Munc-13, tomosyn, snapin, and syntaphilin that bind to individual SNARE proteins) have been suggested to regulate the availability and/or propensity of free SNARE proteins to form functional release machinery ( 19-25).	bind
50560	9	11557	6	10	NULL	0	NULL	complexins			regulates					statement 7		availability of;;propensity of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_24_14038_s_14	11707603	A number of molecules (including Munc18/n-Sec1/rbSec1, complexins, Munc-13, tomosyn, snapin, and syntaphilin that bind to individual SNARE proteins) have been suggested to regulate the availability and/or propensity of free SNARE proteins to form functional release machinery ( 19-25).	bind
50561	10	11557	6	10	NULL	0	NULL	Munc-13			regulates					statement 7		availability of;;propensity of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_24_14038_s_14	11707603	A number of molecules (including Munc18/n-Sec1/rbSec1, complexins, Munc-13, tomosyn, snapin, and syntaphilin that bind to individual SNARE proteins) have been suggested to regulate the availability and/or propensity of free SNARE proteins to form functional release machinery ( 19-25).	bind
50562	11	11557	6	10	NULL	0	NULL	tomosyn			regulates					statement 7		availability of;;propensity of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_24_14038_s_14	11707603	A number of molecules (including Munc18/n-Sec1/rbSec1, complexins, Munc-13, tomosyn, snapin, and syntaphilin that bind to individual SNARE proteins) have been suggested to regulate the availability and/or propensity of free SNARE proteins to form functional release machinery ( 19-25).	bind
50563	12	11557	6	10	NULL	0	NULL	snapin			regulates					statement 7		availability of;;propensity of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_24_14038_s_14	11707603	A number of molecules (including Munc18/n-Sec1/rbSec1, complexins, Munc-13, tomosyn, snapin, and syntaphilin that bind to individual SNARE proteins) have been suggested to regulate the availability and/or propensity of free SNARE proteins to form functional release machinery ( 19-25).	bind
50564	13	11557	6	10	NULL	0	NULL	syntaphilin			regulates					statement 7		availability of;;propensity of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_24_14038_s_14	11707603	A number of molecules (including Munc18/n-Sec1/rbSec1, complexins, Munc-13, tomosyn, snapin, and syntaphilin that bind to individual SNARE proteins) have been suggested to regulate the availability and/or propensity of free SNARE proteins to form functional release machinery ( 19-25).	bind
51175	1	11558	5	NULL	NULL	NULL	NULL	CDK2 monomer	GP		bind					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1754_1_132_s_201	16271522	A number of monomeric CDK2 and T160-phosphorylated CDK2/cyclin A structures are available  bound to ATP or ATP-competitive CDK2-selective inhibitors which can be analysed to  determine which residues lie within 5  Ang  of any ligand atom.	bind
51176	2	11558	5	NULL	NULL	NULL	NULL	CDK2 monomer	GP		bind					CDK2-selective inhibitors	Chemical	ATP-competitive			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1754_1_132_s_201	16271522	A number of monomeric CDK2 and T160-phosphorylated CDK2/cyclin A structures are available  bound to ATP or ATP-competitive CDK2-selective inhibitors which can be analysed to  determine which residues lie within 5  Ang  of any ligand atom.	bind
51177	3	11558	5	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1754_1_132_s_201	16271522	A number of monomeric CDK2 and T160-phosphorylated CDK2/cyclin A structures are available  bound to ATP or ATP-competitive CDK2-selective inhibitors which can be analysed to  determine which residues lie within 5  Ang  of any ligand atom.	bind
51178	4	11558	5	NULL	NULL	NULL	NULL	CDK2/cyclin A	GP	phosphorylated	bind			T160		ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1754_1_132_s_201	16271522	A number of monomeric CDK2 and T160-phosphorylated CDK2/cyclin A structures are available  bound to ATP or ATP-competitive CDK2-selective inhibitors which can be analysed to  determine which residues lie within 5  Ang  of any ligand atom.	bind
51179	5	11558	5	NULL	NULL	NULL	NULL	CDK2/cyclin A	GP	phosphorylated	bind			T160		CDK2-selective inhibitors	Chemical	ATP-competitive			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1754_1_132_s_201	16271522	A number of monomeric CDK2 and T160-phosphorylated CDK2/cyclin A structures are available  bound to ATP or ATP-competitive CDK2-selective inhibitors which can be analysed to  determine which residues lie within 5  Ang  of any ligand atom.	bind
51180	6	11558	5	NULL	NULL	NULL	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1754_1_132_s_201	16271522	A number of monomeric CDK2 and T160-phosphorylated CDK2/cyclin A structures are available  bound to ATP or ATP-competitive CDK2-selective inhibitors which can be analysed to  determine which residues lie within 5  Ang  of any ligand atom.	bind
50566	1	11558	6	NULL	NULL	0	NULL	CDK2	NULL		bind	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1754_1_132_s_201	16271522	A number of monomeric CDK2 and T160-phosphorylated CDK2/cyclin A structures are available  bound to ATP or ATP-competitive CDK2-selective inhibitors which can be analysed to  determine which residues lie within 5  Ang  of any ligand atom.	bind
50567	2	11558	6	NULL	NULL	0	NULL	CDK2/cyclin A	NULL	phosphorylated	bind	NULL		T160		ATP	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1754_1_132_s_201	16271522	A number of monomeric CDK2 and T160-phosphorylated CDK2/cyclin A structures are available  bound to ATP or ATP-competitive CDK2-selective inhibitors which can be analysed to  determine which residues lie within 5  Ang  of any ligand atom.	bind
50568	3	11558	6	NULL	NULL	0	NULL	CDK2	NULL		bind	NULL				CDK2-selective inhibitors	NULL	ATP-competitive			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1754_1_132_s_201	16271522	A number of monomeric CDK2 and T160-phosphorylated CDK2/cyclin A structures are available  bound to ATP or ATP-competitive CDK2-selective inhibitors which can be analysed to  determine which residues lie within 5  Ang  of any ligand atom.	bind
50569	4	11558	6	NULL	NULL	0	NULL	CDK2/cyclin A	NULL	phosphorylated	bind	NULL		T160		CDK2-selective inhibitors	NULL	ATP-competitive			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1754_1_132_s_201	16271522	A number of monomeric CDK2 and T160-phosphorylated CDK2/cyclin A structures are available  bound to ATP or ATP-competitive CDK2-selective inhibitors which can be analysed to  determine which residues lie within 5  Ang  of any ligand atom.	bind
50570	5	11558	6	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1754_1_132_s_201	16271522	A number of monomeric CDK2 and T160-phosphorylated CDK2/cyclin A structures are available  bound to ATP or ATP-competitive CDK2-selective inhibitors which can be analysed to  determine which residues lie within 5  Ang  of any ligand atom.	bind
50571	6	11558	6	NULL	NULL	0	NULL	statement 2	NULL		is an alternative to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1754_1_132_s_201	16271522	A number of monomeric CDK2 and T160-phosphorylated CDK2/cyclin A structures are available  bound to ATP or ATP-competitive CDK2-selective inhibitors which can be analysed to  determine which residues lie within 5  Ang  of any ligand atom.	bind
51181	1	11560	5	NULL	NULL	NULL	NULL			mutant	alter			beta2AR tail		receptors	GP	endocytic membrane trafficking of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_5_3305_s_26	15548537	A number of mutations of the beta2AR tail that alter the endocytic membrane trafficking of receptors also disrupt receptor interaction with NSF, and  in vitro studies indicate that NSF and PDZ proteins bind to the beta2AR tail competitively.	bind
51183	3	11560	5	NULL	NULL	NULL	NULL			mutant	disrupt			beta2AR tail		statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_5_3305_s_26	15548537	A number of mutations of the beta2AR tail that alter the endocytic membrane trafficking of receptors also disrupt receptor interaction with NSF, and  in vitro studies indicate that NSF and PDZ proteins bind to the beta2AR tail competitively.	bind
51184	2	11560	5	NULL	NULL	NULL	NULL	NSF proteins	GP		bind								beta2AR tail		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_5_3305_s_26	15548537	A number of mutations of the beta2AR tail that alter the endocytic membrane trafficking of receptors also disrupt receptor interaction with NSF, and  in vitro studies indicate that NSF and PDZ proteins bind to the beta2AR tail competitively.	bind
51185	4	11560	5	NULL	NULL	NULL	NULL	PDZ proteins	GP		bind								beta2AR tail		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_5_3305_s_26	15548537	A number of mutations of the beta2AR tail that alter the endocytic membrane trafficking of receptors also disrupt receptor interaction with NSF, and  in vitro studies indicate that NSF and PDZ proteins bind to the beta2AR tail competitively.	bind
51186	5	11560	5	NULL	NULL	NULL	NULL	statement 2	Process		competes with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_5_3305_s_26	15548537	A number of mutations of the beta2AR tail that alter the endocytic membrane trafficking of receptors also disrupt receptor interaction with NSF, and  in vitro studies indicate that NSF and PDZ proteins bind to the beta2AR tail competitively.	bind
50579	1	11560	6	NULL	NULL	0	NULL	NSF	NULL		bind	NULL					NULL		beta2AR tail		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_5_3305_s_26	15548537	A number of mutations of the beta2AR tail that alter the endocytic membrane trafficking of receptors also disrupt receptor interaction with NSF, and  in vitro studies indicate that NSF and PDZ proteins bind to the beta2AR tail competitively.	bind
50580	2	11560	6	NULL	NULL	0	NULL	PDZ protein	NULL		bind	NULL					NULL		beta2AR tail		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_5_3305_s_26	15548537	A number of mutations of the beta2AR tail that alter the endocytic membrane trafficking of receptors also disrupt receptor interaction with NSF, and  in vitro studies indicate that NSF and PDZ proteins bind to the beta2AR tail competitively.	bind
50581	3	11560	6	NULL	NULL	0	NULL	statement 1	NULL		competes	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_5_3305_s_26	15548537	A number of mutations of the beta2AR tail that alter the endocytic membrane trafficking of receptors also disrupt receptor interaction with NSF, and  in vitro studies indicate that NSF and PDZ proteins bind to the beta2AR tail competitively.	bind
50582	4	11560	6	NULL	NULL	0	NULL		NULL	mutation of	alters	NULL		beta2AR tail		receptor	NULL	endocytic membrane trafficking of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_5_3305_s_26	15548537	A number of mutations of the beta2AR tail that alter the endocytic membrane trafficking of receptors also disrupt receptor interaction with NSF, and  in vitro studies indicate that NSF and PDZ proteins bind to the beta2AR tail competitively.	bind
50583	5	11560	6	NULL	NULL	0	NULL		NULL	mutation of	disrupts	NULL		beta2AR tail		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_5_3305_s_26	15548537	A number of mutations of the beta2AR tail that alter the endocytic membrane trafficking of receptors also disrupt receptor interaction with NSF, and  in vitro studies indicate that NSF and PDZ proteins bind to the beta2AR tail competitively.	bind
51187	1	11561	5	NULL	NULL	NULL	NULL	nAChR agonists	GP		bind					alpha4/beta2 receptor	GP				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jneurosci_20_17_6431_s_19	10964949	A number of nAChR agonists that bind to the alpha4/beta2 receptor configuration  in vitro are known to have an effect on anxiety (Pomerleau, 1986  ; Gilbert et al., 1989  ; Brioni et al., 1993  ), attention (Brioni et al., 1997  ), and antinociception (Tripathi et al., 1982  ; Damaj et al., 1998  ), implicating the alpha4/beta2 receptor in the mediation of a number of physiological processes.	bind
51188	2	11561	5	NULL	NULL	NULL	NULL	statement 1	Process		effects					anxiety	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_20_17_6431_s_19	10964949	A number of nAChR agonists that bind to the alpha4/beta2 receptor configuration  in vitro are known to have an effect on anxiety (Pomerleau, 1986  ; Gilbert et al., 1989  ; Brioni et al., 1993  ), attention (Brioni et al., 1997  ), and antinociception (Tripathi et al., 1982  ; Damaj et al., 1998  ), implicating the alpha4/beta2 receptor in the mediation of a number of physiological processes.	bind
51189	3	11561	5	NULL	NULL	NULL	NULL	statement 1	Process		effects					attention	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_20_17_6431_s_19	10964949	A number of nAChR agonists that bind to the alpha4/beta2 receptor configuration  in vitro are known to have an effect on anxiety (Pomerleau, 1986  ; Gilbert et al., 1989  ; Brioni et al., 1993  ), attention (Brioni et al., 1997  ), and antinociception (Tripathi et al., 1982  ; Damaj et al., 1998  ), implicating the alpha4/beta2 receptor in the mediation of a number of physiological processes.	bind
51190	4	11561	5	NULL	NULL	NULL	NULL	statement 1	Process		effects					antinociception	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_20_17_6431_s_19	10964949	A number of nAChR agonists that bind to the alpha4/beta2 receptor configuration  in vitro are known to have an effect on anxiety (Pomerleau, 1986  ; Gilbert et al., 1989  ; Brioni et al., 1993  ), attention (Brioni et al., 1997  ), and antinociception (Tripathi et al., 1982  ; Damaj et al., 1998  ), implicating the alpha4/beta2 receptor in the mediation of a number of physiological processes.	bind
50584	1	11561	6	NULL	NULL	0	NULL	nAChR agonists	NULL		bind	NULL				alpha4/beta2 receptor	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_jneurosci_20_17_6431_s_19	10964949	A number of nAChR agonists that bind to the alpha4/beta2 receptor configuration  in vitro are known to have an effect on anxiety (Pomerleau, 1986  ; Gilbert et al., 1989  ; Brioni et al., 1993  ), attention (Brioni et al., 1997  ), and antinociception (Tripathi et al., 1982  ; Damaj et al., 1998  ), implicating the alpha4/beta2 receptor in the mediation of a number of physiological processes.	bind
50585	2	11561	6	NULL	NULL	0	NULL	nAChR agonists	NULL		plays a role in	NULL				anxiety	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_17_6431_s_19	10964949	A number of nAChR agonists that bind to the alpha4/beta2 receptor configuration  in vitro are known to have an effect on anxiety (Pomerleau, 1986  ; Gilbert et al., 1989  ; Brioni et al., 1993  ), attention (Brioni et al., 1997  ), and antinociception (Tripathi et al., 1982  ; Damaj et al., 1998  ), implicating the alpha4/beta2 receptor in the mediation of a number of physiological processes.	bind
50586	3	11561	6	NULL	NULL	0	NULL	nAChR agonists	NULL		plays a role in	NULL				attention	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_17_6431_s_19	10964949	A number of nAChR agonists that bind to the alpha4/beta2 receptor configuration  in vitro are known to have an effect on anxiety (Pomerleau, 1986  ; Gilbert et al., 1989  ; Brioni et al., 1993  ), attention (Brioni et al., 1997  ), and antinociception (Tripathi et al., 1982  ; Damaj et al., 1998  ), implicating the alpha4/beta2 receptor in the mediation of a number of physiological processes.	bind
50587	4	11561	6	NULL	NULL	0	NULL	nAChR agonists	NULL		plays a role in	NULL				antinociception	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_17_6431_s_19	10964949	A number of nAChR agonists that bind to the alpha4/beta2 receptor configuration  in vitro are known to have an effect on anxiety (Pomerleau, 1986  ; Gilbert et al., 1989  ; Brioni et al., 1993  ), attention (Brioni et al., 1997  ), and antinociception (Tripathi et al., 1982  ; Damaj et al., 1998  ), implicating the alpha4/beta2 receptor in the mediation of a number of physiological processes.	bind
51191	1	11562	5	NULL	NULL	0	NULL		NULL		surround	NULL			negative elements		NULL			2L exon	NULL		0	NULL	NULL	NULL	gw60_neuron_25_2_359_s_291	10719891	A number of negative elements surrounding the  2L exon were found to bind PTB, and evidence was also found for positive acting splicing elements.	bind
51192	2	11562	5	NULL	NULL	NULL	NULL	statement 1	NucleicAcid		bind					PTB	GP				NULL		NULL	NULL	NULL	NULL	gw60_neuron_25_2_359_s_291	10719891	A number of negative elements surrounding the  2L exon were found to bind PTB, and evidence was also found for positive acting splicing elements.	bind
50588	1	11562	6	10	NULL	0	NULL				surround				negative elements	2L exon					NULL		NULL	NULL	NULL	NULL	gw60_neuron_25_2_359_s_291	10719891	A number of negative elements surrounding the  2L exon were found to bind PTB, and evidence was also found for positive acting splicing elements.	bind
50589	2	11562	6	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL				PTB	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_25_2_359_s_291	10719891	A number of negative elements surrounding the  2L exon were found to bind PTB, and evidence was also found for positive acting splicing elements.	bind
51193	1	11563	5	NULL	NULL	NULL	NULL	bZIP	GP		is a superfamily of 					transcription factors	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2500_s_35	8999965	A number of nuclear proteins specifically bind to the CRE and CRE-like sequences ( 25), and these are all members of the bZIP superfamily of transcription factors.	bind
51194	2	11563	5	NULL	NULL	NULL	NULL	bZIP	GP		bind		specifically							CRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2500_s_35	8999965	A number of nuclear proteins specifically bind to the CRE and CRE-like sequences ( 25), and these are all members of the bZIP superfamily of transcription factors.	bind
51195	3	11563	5	NULL	NULL	NULL	NULL	bZIP	GP		bind		specifically							CRE-like sequences	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2500_s_35	8999965	A number of nuclear proteins specifically bind to the CRE and CRE-like sequences ( 25), and these are all members of the bZIP superfamily of transcription factors.	bind
50590	1	11563	6	10	NULL	0	NULL	bZIP 			bind		specifically							CRE	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2500_s_35	8999965	A number of nuclear proteins specifically bind to the CRE and CRE-like sequences ( 25), and these are all members of the bZIP superfamily of transcription factors.	bind
50591	2	11563	6	10	NULL	0	NULL	bZIP			bind		specifically							CRE-like sequences	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_4_2500_s_35	8999965	A number of nuclear proteins specifically bind to the CRE and CRE-like sequences ( 25), and these are all members of the bZIP superfamily of transcription factors.	bind
54198	3	11563	6	10	NULL	0	NULL	bZIP			is a superfamily of					transcription factors					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_4_2500_s_35	8999965	A number of nuclear proteins specifically bind to the CRE and CRE-like sequences ( 25), and these are all members of the bZIP superfamily of transcription factors.	bind
51196	1	11564	5	NULL	NULL	NULL	NULL	TL	GP		bind					rifampin	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1688_2_102_s_33	14990340	A number of observations led to the hypothesis that TL would bind rifampin with higher  affinity than albumin.	bind
51197	2	11564	5	NULL	NULL	NULL	NULL	TL	GP		bind					albumin	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1688_2_102_s_33	14990340	A number of observations led to the hypothesis that TL would bind rifampin with higher  affinity than albumin.	bind
51198	3	11564	5	NULL	NULL	NULL	NULL	statement 1	Process	affinity of	is higher than					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1688_2_102_s_33	14990340	A number of observations led to the hypothesis that TL would bind rifampin with higher  affinity than albumin.	bind
50592	1	11564	6	NULL	NULL	0	NULL	TL	NULL		bind	NULL				rifampin	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1688_2_102_s_33	14990340	A number of observations led to the hypothesis that TL would bind rifampin with higher  affinity than albumin.	bind
50593	2	11564	6	NULL	NULL	0	NULL	TL	NULL		bind	NULL				albumin	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1688_2_102_s_33	14990340	A number of observations led to the hypothesis that TL would bind rifampin with higher  affinity than albumin.	bind
50594	3	11564	6	10	NULL	0	NULL	statement 1		affinity of	is higher than					statement 2		affinity of			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1688_2_102_s_33	14990340	A number of observations led to the hypothesis that TL would bind rifampin with higher  affinity than albumin.	bind
51203	1	11565	5	NULL	NULL	NULL	NULL	mAb 220	GP		reacts with					Equ c 1	GP	natural			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_28_21572_s_179	10787420	A number of observations provides further insight on candidate regions for the putative binding targets of human IgE and mouse mAb 220 in Equ c 1: (i) the epitopes are unlikely to include a protein-bound carbohydrate because mAb 220 and IgE serum display a similar reactivity for natural and recombinant Equ c 1	bind
51204	2	11565	5	NULL	NULL	NULL	NULL	mAb 220	GP		reacts with					Equ c 1	GP	recombinant			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_28_21572_s_179	10787420	A number of observations provides further insight on candidate regions for the putative binding targets of human IgE and mouse mAb 220 in Equ c 1: (i) the epitopes are unlikely to include a protein-bound carbohydrate because mAb 220 and IgE serum display a similar reactivity for natural and recombinant Equ c 1	bind
51205	3	11565	5	NULL	NULL	NULL	NULL	IgE serum	CellComponent		reacts with					Equ c 1	GP	natural			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_28_21572_s_179	10787420	A number of observations provides further insight on candidate regions for the putative binding targets of human IgE and mouse mAb 220 in Equ c 1: (i) the epitopes are unlikely to include a protein-bound carbohydrate because mAb 220 and IgE serum display a similar reactivity for natural and recombinant Equ c 1	bind
51206	4	11565	5	NULL	NULL	NULL	NULL	IgE serum	CellComponent		reacts with					Equ c 1	GP	recombinant			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_28_21572_s_179	10787420	A number of observations provides further insight on candidate regions for the putative binding targets of human IgE and mouse mAb 220 in Equ c 1: (i) the epitopes are unlikely to include a protein-bound carbohydrate because mAb 220 and IgE serum display a similar reactivity for natural and recombinant Equ c 1	bind
50595	1	11565	6	NULL	NULL	0	NULL	mAb 220	NULL		reacts with	NULL				Equ c 1	NULL	natural			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_28_21572_s_179	10787420	A number of observations provides further insight on candidate regions for the putative binding targets of human IgE and mouse mAb 220 in Equ c 1: (i) the epitopes are unlikely to include a protein-bound carbohydrate because mAb 220 and IgE serum display a similar reactivity for natural and recombinant Equ c 1	bind
50596	2	11565	6	NULL	NULL	0	NULL	mAb 220	NULL		reacts with	NULL				Equ c 1	NULL	recombinant			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_28_21572_s_179	10787420	A number of observations provides further insight on candidate regions for the putative binding targets of human IgE and mouse mAb 220 in Equ c 1: (i) the epitopes are unlikely to include a protein-bound carbohydrate because mAb 220 and IgE serum display a similar reactivity for natural and recombinant Equ c 1	bind
50597	3	11565	6	NULL	NULL	0	NULL	IgE serum	NULL		reacts with	NULL				Equ c 1	NULL	natural			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_28_21572_s_179	10787420	A number of observations provides further insight on candidate regions for the putative binding targets of human IgE and mouse mAb 220 in Equ c 1: (i) the epitopes are unlikely to include a protein-bound carbohydrate because mAb 220 and IgE serum display a similar reactivity for natural and recombinant Equ c 1	bind
50598	4	11565	6	NULL	NULL	0	NULL	IgE serum	NULL		reacts with	NULL				Equ c 1	NULL	recombinant			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_28_21572_s_179	10787420	A number of observations provides further insight on candidate regions for the putative binding targets of human IgE and mouse mAb 220 in Equ c 1: (i) the epitopes are unlikely to include a protein-bound carbohydrate because mAb 220 and IgE serum display a similar reactivity for natural and recombinant Equ c 1	bind
51199	1	11566	5	NULL	NULL	NULL	NULL	ADAMTS-1	GP		bind					ECM components	AbstractConcept				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_11_10109_s_310	14662755	A number of other ADAMTSs, including ADAMTS-1 ( ,  ), ADAMTS-5 ( ,  ), and ADAMTS-9 ( ) bind to ECM components, but not ADAMTS-13 ( ).	bind
51200	2	11566	5	NULL	NULL	NULL	NULL	ADAMTS-5	GP		bind					ECM components	AbstractConcept				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_11_10109_s_310	14662755	A number of other ADAMTSs, including ADAMTS-1 ( ,  ), ADAMTS-5 ( ,  ), and ADAMTS-9 ( ) bind to ECM components, but not ADAMTS-13 ( ).	bind
51201	3	11566	5	NULL	NULL	NULL	NULL	ADAMTS-9	GP		bind					ECM components	AbstractConcept				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_11_10109_s_310	14662755	A number of other ADAMTSs, including ADAMTS-1 ( ,  ), ADAMTS-5 ( ,  ), and ADAMTS-9 ( ) bind to ECM components, but not ADAMTS-13 ( ).	bind
51202	4	11566	5	NULL	NULL	NULL	NULL	ADAMTS-13	GP		does not bind					ECM components	AbstractConcept				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_11_10109_s_310	14662755	A number of other ADAMTSs, including ADAMTS-1 ( ,  ), ADAMTS-5 ( ,  ), and ADAMTS-9 ( ) bind to ECM components, but not ADAMTS-13 ( ).	bind
50599	1	11566	6	NULL	NULL	0	NULL	ADAMTS-1	NULL		bind	NULL				ECM components	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_11_10109_s_310	14662755	A number of other ADAMTSs, including ADAMTS-1 ( ,  ), ADAMTS-5 ( ,  ), and ADAMTS-9 ( ) bind to ECM components, but not ADAMTS-13 ( ).	bind
50600	2	11566	6	NULL	NULL	0	NULL	ADAMTS-5	NULL		bind	NULL				ECM components	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_11_10109_s_310	14662755	A number of other ADAMTSs, including ADAMTS-1 ( ,  ), ADAMTS-5 ( ,  ), and ADAMTS-9 ( ) bind to ECM components, but not ADAMTS-13 ( ).	bind
50601	3	11566	6	NULL	NULL	0	NULL	ADAMTS-9	NULL		bind	NULL				ECM components	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_11_10109_s_310	14662755	A number of other ADAMTSs, including ADAMTS-1 ( ,  ), ADAMTS-5 ( ,  ), and ADAMTS-9 ( ) bind to ECM components, but not ADAMTS-13 ( ).	bind
50602	4	11566	6	NULL	NULL	0	NULL	ADAMTS-13	NULL		does not bind	NULL				ECM components	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_11_10109_s_310	14662755	A number of other ADAMTSs, including ADAMTS-1 ( ,  ), ADAMTS-5 ( ,  ), and ADAMTS-9 ( ) bind to ECM components, but not ADAMTS-13 ( ).	bind
51210	1	11567	5	NULL	NULL	NULL	NULL	STAT2	GP		bind					p300/CBP-CH1	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_13_1_64_s_295	9887100	A number of other factors, e.g., STAT2 (Bhattacharya et al. 1996  ), ets-1 (Yang et al. 1998  ), NFkappaB-p65 (Zhong et al. 1998  ), p53, and MDM2 (Grossman et al. 1998  ) bind to p300/CBP-CH1, and could occupy available binding sites.	bind
51211	2	11567	5	NULL	NULL	NULL	NULL	ets-1	GP		bind					p300/CBP-CH1	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_13_1_64_s_295	9887100	A number of other factors, e.g., STAT2 (Bhattacharya et al. 1996  ), ets-1 (Yang et al. 1998  ), NFkappaB-p65 (Zhong et al. 1998  ), p53, and MDM2 (Grossman et al. 1998  ) bind to p300/CBP-CH1, and could occupy available binding sites.	bind
51212	3	11567	5	NULL	NULL	NULL	NULL	NFkappaB-p65	GP		bind					p300/CBP-CH1	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_13_1_64_s_295	9887100	A number of other factors, e.g., STAT2 (Bhattacharya et al. 1996  ), ets-1 (Yang et al. 1998  ), NFkappaB-p65 (Zhong et al. 1998  ), p53, and MDM2 (Grossman et al. 1998  ) bind to p300/CBP-CH1, and could occupy available binding sites.	bind
51213	4	11567	5	NULL	NULL	NULL	NULL	p53	GP		bind					p300/CBP-CH1	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_13_1_64_s_295	9887100	A number of other factors, e.g., STAT2 (Bhattacharya et al. 1996  ), ets-1 (Yang et al. 1998  ), NFkappaB-p65 (Zhong et al. 1998  ), p53, and MDM2 (Grossman et al. 1998  ) bind to p300/CBP-CH1, and could occupy available binding sites.	bind
51214	5	11567	5	NULL	NULL	NULL	NULL	MDM2	GP		bind					p300/CBP-CH1	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_13_1_64_s_295	9887100	A number of other factors, e.g., STAT2 (Bhattacharya et al. 1996  ), ets-1 (Yang et al. 1998  ), NFkappaB-p65 (Zhong et al. 1998  ), p53, and MDM2 (Grossman et al. 1998  ) bind to p300/CBP-CH1, and could occupy available binding sites.	bind
50603	1	11567	6	NULL	NULL	0	NULL	STAT2	NULL		bind	NULL				p300/CBP-CH1	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_13_1_64_s_295	9887100	A number of other factors, e.g., STAT2 (Bhattacharya et al. 1996  ), ets-1 (Yang et al. 1998  ), NFkappaB-p65 (Zhong et al. 1998  ), p53, and MDM2 (Grossman et al. 1998  ) bind to p300/CBP-CH1, and could occupy available binding sites.	bind
50604	2	11567	6	NULL	NULL	0	NULL	ets-1	NULL		bind	NULL				p300/CBP-CH1	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_13_1_64_s_295	9887100	A number of other factors, e.g., STAT2 (Bhattacharya et al. 1996  ), ets-1 (Yang et al. 1998  ), NFkappaB-p65 (Zhong et al. 1998  ), p53, and MDM2 (Grossman et al. 1998  ) bind to p300/CBP-CH1, and could occupy available binding sites.	bind
50605	3	11567	6	NULL	NULL	0	NULL	NFkappaB-p65	NULL		bind	NULL				p300/CBP-CH1	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_13_1_64_s_295	9887100	A number of other factors, e.g., STAT2 (Bhattacharya et al. 1996  ), ets-1 (Yang et al. 1998  ), NFkappaB-p65 (Zhong et al. 1998  ), p53, and MDM2 (Grossman et al. 1998  ) bind to p300/CBP-CH1, and could occupy available binding sites.	bind
50606	4	11567	6	NULL	NULL	0	NULL	p53	NULL		bind	NULL				p300/CBP-CH1	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_13_1_64_s_295	9887100	A number of other factors, e.g., STAT2 (Bhattacharya et al. 1996  ), ets-1 (Yang et al. 1998  ), NFkappaB-p65 (Zhong et al. 1998  ), p53, and MDM2 (Grossman et al. 1998  ) bind to p300/CBP-CH1, and could occupy available binding sites.	bind
50607	5	11567	6	NULL	NULL	0	NULL	MDM2	NULL		bind	NULL				p300/CBP-CH1	NULL				NULL		0	NULL	NULL	NULL	gw60_genesdev_13_1_64_s_295	9887100	A number of other factors, e.g., STAT2 (Bhattacharya et al. 1996  ), ets-1 (Yang et al. 1998  ), NFkappaB-p65 (Zhong et al. 1998  ), p53, and MDM2 (Grossman et al. 1998  ) bind to p300/CBP-CH1, and could occupy available binding sites.	bind
51215	1	11569	5	NULL	NULL	NULL	NULL	IGF-I	GP		bind					insulin receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_443_3_271_s_16	10025946	A number of papers report the different activities of these seven binding proteins including regulating half-life in circulation, transporting IGF-I to specific tissues, preventing hypoglycemia by inhibiting the binding of IGF-I to the insulin receptor  [ 10,   11] and mediating p53-induced cell cycle arrest  [ 12,   13].	bind
51216	2	11569	5	NULL	NULL	NULL	NULL	p53	GP		induce					cell cycle arrest	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_443_3_271_s_16	10025946	A number of papers report the different activities of these seven binding proteins including regulating half-life in circulation, transporting IGF-I to specific tissues, preventing hypoglycemia by inhibiting the binding of IGF-I to the insulin receptor  [ 10,   11] and mediating p53-induced cell cycle arrest  [ 12,   13].	bind
51226	3	11569	5	NULL	NULL	NULL	NULL	statement 1	Process	inhibition of	prevents					hypoglycemia	MedicalFinding				NULL		NULL	NULL	NULL	NULL	gw60_febslett_443_3_271_s_16	10025946	A number of papers report the different activities of these seven binding proteins including regulating half-life in circulation, transporting IGF-I to specific tissues, preventing hypoglycemia by inhibiting the binding of IGF-I to the insulin receptor  [ 10,   11] and mediating p53-induced cell cycle arrest  [ 12,   13].	bind
50608	1	11569	6	NULL	NULL	0	NULL	IGF-I	NULL		bind	NULL				insulin receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_443_3_271_s_16	10025946	A number of papers report the different activities of these seven binding proteins including regulating half-life in circulation, transporting IGF-I to specific tissues, preventing hypoglycemia by inhibiting the binding of IGF-I to the insulin receptor  [ 10,   11] and mediating p53-induced cell cycle arrest  [ 12,   13].	bind
50609	2	11569	6	NULL	NULL	0	NULL	p53	NULL		induces	NULL				cell cycle arrest	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_443_3_271_s_16	10025946	A number of papers report the different activities of these seven binding proteins including regulating half-life in circulation, transporting IGF-I to specific tissues, preventing hypoglycemia by inhibiting the binding of IGF-I to the insulin receptor  [ 10,   11] and mediating p53-induced cell cycle arrest  [ 12,   13].	bind
54199	3	11569	6	10	NULL	0	NULL	statement 1		inhibition of	prevents					hypoglycemia					NULL		0	NULL	NULL	NULL	gw60_febslett_443_3_271_s_16	10025946	A number of papers report the different activities of these seven binding proteins including regulating half-life in circulation, transporting IGF-I to specific tissues, preventing hypoglycemia by inhibiting the binding of IGF-I to the insulin receptor  [ 10,   11] and mediating p53-induced cell cycle arrest  [ 12,   13].	bind
51227	1	11570	5	NULL	NULL	NULL	NULL	pathogenic microbes	Organism		bind					fH	GP				NULL	in vivo	NULL	NULL	NULL	NULL	abs-batch0700-0719_j-immunol_176_12_16751403_s_4	16751403	A number of pathogenic microbes bind factor H (fH),  the negative regulator of the alternative pathway of complement activation,  to promote their survival in vivo.	bind
51228	2	11570	5	NULL	NULL	NULL	NULL	fH	GP		is					factor H	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_j-immunol_176_12_16751403_s_4	16751403	A number of pathogenic microbes bind factor H (fH),  the negative regulator of the alternative pathway of complement activation,  to promote their survival in vivo.	bind
51229	3	11570	5	NULL	NULL	NULL	NULL	fH	GP		regulates		negatively			complement 	GP	alternative pathway of ;;activation of			NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_j-immunol_176_12_16751403_s_4	16751403	A number of pathogenic microbes bind factor H (fH),  the negative regulator of the alternative pathway of complement activation,  to promote their survival in vivo.	bind
51230	4	11570	5	NULL	NULL	NULL	NULL	statement 1	Process		promotes					pathogenic microbes	Organism	survival of			NULL	in vivo	NULL	NULL	NULL	NULL	abs-batch0700-0719_j-immunol_176_12_16751403_s_4	16751403	A number of pathogenic microbes bind factor H (fH),  the negative regulator of the alternative pathway of complement activation,  to promote their survival in vivo.	bind
50610	1	11570	6	NULL	NULL	0	NULL	pathogenic microbes	NULL		bind	NULL				factor H	NULL				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_j-immunol_176_12_16751403_s_4	16751403	A number of pathogenic microbes bind factor H (fH),  the negative regulator of the alternative pathway of complement activation,  to promote their survival in vivo.	bind
50611	2	11570	6	NULL	NULL	0	NULL	fH	NULL		is	NULL				factor H	NULL				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_j-immunol_176_12_16751403_s_4	16751403	A number of pathogenic microbes bind factor H (fH),  the negative regulator of the alternative pathway of complement activation,  to promote their survival in vivo.	bind
50612	3	11570	6	10	NULL	0	NULL	fH			regulates		negatively 			complement		alternative pathway of ;;activation of			NULL		NULL	NULL	NULL	NULL	abs-batch0700-0719_j-immunol_176_12_16751403_s_4	16751403	A number of pathogenic microbes bind factor H (fH),  the negative regulator of the alternative pathway of complement activation,  to promote their survival in vivo.	bind
54200	4	11570	6	10	NULL	0	NULL	statement 1			promote					pathogenic microbes		survival of			NULL	in vivo	NULL	NULL	NULL	NULL	abs-batch0700-0719_j-immunol_176_12_16751403_s_4	16751403	A number of pathogenic microbes bind factor H (fH),  the negative regulator of the alternative pathway of complement activation,  to promote their survival in vivo.	bind
51231	1	11572	5	NULL	NULL	NULL	NULL	GPIa-IIa	GP		interacts with					collagen	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevmed_52_0_161_s_37	11160773	A number of platelet proteins interact with collagen besides  2 1 (GPIa-IIa), including   IIb (GPIIb), GPIV, GPVI, and two other proteins: a 65,000-molecular-weight protein  that binds to type I collagen and an 85-90,000-molecular-weight protein ( 9).	bind
51232	2	11572	5	NULL	NULL	NULL	NULL	GPIIb	GP		interacts with					collagen	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevmed_52_0_161_s_37	11160773	A number of platelet proteins interact with collagen besides  2 1 (GPIa-IIa), including   IIb (GPIIb), GPIV, GPVI, and two other proteins: a 65,000-molecular-weight protein  that binds to type I collagen and an 85-90,000-molecular-weight protein ( 9).	bind
51233	3	11572	5	NULL	NULL	NULL	NULL	GPIV	GP		interacts with					collagen	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevmed_52_0_161_s_37	11160773	A number of platelet proteins interact with collagen besides  2 1 (GPIa-IIa), including   IIb (GPIIb), GPIV, GPVI, and two other proteins: a 65,000-molecular-weight protein  that binds to type I collagen and an 85-90,000-molecular-weight protein ( 9).	bind
51234	4	11572	5	NULL	NULL	NULL	NULL	GPVI	GP		interacts with					collagen	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevmed_52_0_161_s_37	11160773	A number of platelet proteins interact with collagen besides  2 1 (GPIa-IIa), including   IIb (GPIIb), GPIV, GPVI, and two other proteins: a 65,000-molecular-weight protein  that binds to type I collagen and an 85-90,000-molecular-weight protein ( 9).	bind
51235	5	11572	5	NULL	NULL	NULL	NULL	GPIa-IIa	GP		is a type of					platelet protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevmed_52_0_161_s_37	11160773	A number of platelet proteins interact with collagen besides  2 1 (GPIa-IIa), including   IIb (GPIIb), GPIV, GPVI, and two other proteins: a 65,000-molecular-weight protein  that binds to type I collagen and an 85-90,000-molecular-weight protein ( 9).	bind
51236	6	11572	5	NULL	NULL	NULL	NULL	GPIIb	GP		is a type of					platelet protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevmed_52_0_161_s_37	11160773	A number of platelet proteins interact with collagen besides  2 1 (GPIa-IIa), including   IIb (GPIIb), GPIV, GPVI, and two other proteins: a 65,000-molecular-weight protein  that binds to type I collagen and an 85-90,000-molecular-weight protein ( 9).	bind
51237	7	11572	5	NULL	NULL	NULL	NULL	GPIV	GP		is a type of					platelet protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevmed_52_0_161_s_37	11160773	A number of platelet proteins interact with collagen besides  2 1 (GPIa-IIa), including   IIb (GPIIb), GPIV, GPVI, and two other proteins: a 65,000-molecular-weight protein  that binds to type I collagen and an 85-90,000-molecular-weight protein ( 9).	bind
51238	8	11572	5	NULL	NULL	NULL	NULL	GPVI	GP		is a type of					platelet protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevmed_52_0_161_s_37	11160773	A number of platelet proteins interact with collagen besides  2 1 (GPIa-IIa), including   IIb (GPIIb), GPIV, GPVI, and two other proteins: a 65,000-molecular-weight protein  that binds to type I collagen and an 85-90,000-molecular-weight protein ( 9).	bind
51240	9	11572	5	NULL	NULL	NULL	NULL	65,000 molecular-weight protein	GP		bind					type I collagen	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevmed_52_0_161_s_37	11160773	A number of platelet proteins interact with collagen besides  2 1 (GPIa-IIa), including   IIb (GPIIb), GPIV, GPVI, and two other proteins: a 65,000-molecular-weight protein  that binds to type I collagen and an 85-90,000-molecular-weight protein ( 9).	bind
50749	1	11572	6	10	NULL	0	NULL	65,000 molecular-weight protein			bind					type I collagen					NULL		NULL	NULL	NULL	NULL	gw70_annurevmed_52_0_161_s_37	11160773	A number of platelet proteins interact with collagen besides  2 1 (GPIa-IIa), including   IIb (GPIIb), GPIV, GPVI, and two other proteins: a 65,000-molecular-weight protein  that binds to type I collagen and an 85-90,000-molecular-weight protein ( 9).	bind
50750	2	11572	6	10	NULL	0	NULL	GPIa-IIa			interacts with					collagen					NULL		NULL	NULL	NULL	NULL	gw70_annurevmed_52_0_161_s_37	11160773	A number of platelet proteins interact with collagen besides  2 1 (GPIa-IIa), including   IIb (GPIIb), GPIV, GPVI, and two other proteins: a 65,000-molecular-weight protein  that binds to type I collagen and an 85-90,000-molecular-weight protein ( 9).	bind
50751	3	11572	6	10	NULL	0	NULL	GPIIb			interacts with					collagen					NULL		NULL	NULL	NULL	NULL	gw70_annurevmed_52_0_161_s_37	11160773	A number of platelet proteins interact with collagen besides  2 1 (GPIa-IIa), including   IIb (GPIIb), GPIV, GPVI, and two other proteins: a 65,000-molecular-weight protein  that binds to type I collagen and an 85-90,000-molecular-weight protein ( 9).	bind
50752	4	11572	6	10	NULL	0	NULL	GPIV			interacts with					collagen					NULL		NULL	NULL	NULL	NULL	gw70_annurevmed_52_0_161_s_37	11160773	A number of platelet proteins interact with collagen besides  2 1 (GPIa-IIa), including   IIb (GPIIb), GPIV, GPVI, and two other proteins: a 65,000-molecular-weight protein  that binds to type I collagen and an 85-90,000-molecular-weight protein ( 9).	bind
50753	5	11572	6	10	NULL	0	NULL	GPVI			interacts with					collagen					NULL		NULL	NULL	NULL	NULL	gw70_annurevmed_52_0_161_s_37	11160773	A number of platelet proteins interact with collagen besides  2 1 (GPIa-IIa), including   IIb (GPIIb), GPIV, GPVI, and two other proteins: a 65,000-molecular-weight protein  that binds to type I collagen and an 85-90,000-molecular-weight protein ( 9).	bind
50754	6	11572	6	NULL	NULL	0	NULL	GPIa-IIa	NULL		is a type of	NULL				platelet protein	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevmed_52_0_161_s_37	11160773	A number of platelet proteins interact with collagen besides  2 1 (GPIa-IIa), including   IIb (GPIIb), GPIV, GPVI, and two other proteins: a 65,000-molecular-weight protein  that binds to type I collagen and an 85-90,000-molecular-weight protein ( 9).	bind
50755	7	11572	6	NULL	NULL	0	NULL	GPIIb	NULL		is a type of	NULL				platelet protein	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevmed_52_0_161_s_37	11160773	A number of platelet proteins interact with collagen besides  2 1 (GPIa-IIa), including   IIb (GPIIb), GPIV, GPVI, and two other proteins: a 65,000-molecular-weight protein  that binds to type I collagen and an 85-90,000-molecular-weight protein ( 9).	bind
50756	8	11572	6	NULL	NULL	0	NULL	GPIV	NULL		is a type of	NULL				platelet protein	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevmed_52_0_161_s_37	11160773	A number of platelet proteins interact with collagen besides  2 1 (GPIa-IIa), including   IIb (GPIIb), GPIV, GPVI, and two other proteins: a 65,000-molecular-weight protein  that binds to type I collagen and an 85-90,000-molecular-weight protein ( 9).	bind
50757	9	11572	6	NULL	NULL	0	NULL	GPVI	NULL		is a type of	NULL				platelet protein	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevmed_52_0_161_s_37	11160773	A number of platelet proteins interact with collagen besides  2 1 (GPIa-IIa), including   IIb (GPIIb), GPIV, GPVI, and two other proteins: a 65,000-molecular-weight protein  that binds to type I collagen and an 85-90,000-molecular-weight protein ( 9).	bind
51258	1	11573	5	NULL	NULL	NULL	NULL			positively charged	bind			arginine side chains		substrate	GP		pyrophosphate groups		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_21_20762_s_175	15788389	A number of positively charged arginine side chains bind to the substrate pyrophosphate groups, between which there is a Mg2+ ion coordinated to Asp26.	bind
51259	2	11573	5	NULL	NULL	NULL	NULL	Mg2+ ion	Chemical		is coordinated to								Asp26		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_21_20762_s_175	15788389	A number of positively charged arginine side chains bind to the substrate pyrophosphate groups, between which there is a Mg2+ ion coordinated to Asp26.	bind
50613	1	11573	6	10	NULL	0	NULL			positively charged	bind			arginine side chains		substrate			pyrophosphate groups		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_21_20762_s_175	15788389	A number of positively charged arginine side chains bind to the substrate pyrophosphate groups, between which there is a Mg2+ ion coordinated to Asp26.	bind
50614	2	11573	6	10	NULL	0	NULL	Mg2+ ion 			is coordinated to								Asp26		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_21_20762_s_175	15788389	A number of positively charged arginine side chains bind to the substrate pyrophosphate groups, between which there is a Mg2+ ion coordinated to Asp26.	bind
51260	1	11574	5	NULL	NULL	NULL	NULL	SHC	GP		bind					CBL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_24_14962_s_183	9614102	A number of previous reports have demonstrated GRB2-mediated SHC binding to CBL ( 20,  38,  45).	bind
51261	2	11574	5	NULL	NULL	NULL	NULL	GRB2	GP		mediates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_24_14962_s_183	9614102	A number of previous reports have demonstrated GRB2-mediated SHC binding to CBL ( 20,  38,  45).	bind
50615	1	11574	6	NULL	NULL	0	NULL	SHC	NULL		bind	NULL				CBL	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_24_14962_s_183	9614102	A number of previous reports have demonstrated GRB2-mediated SHC binding to CBL ( 20,  38,  45).	bind
50616	2	11574	6	10	NULL	0	NULL	GRB2			mediates					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_24_14962_s_183	9614102	A number of previous reports have demonstrated GRB2-mediated SHC binding to CBL ( 20,  38,  45).	bind
51262	1	11575	5	NULL	NULL	NULL	NULL	Mlp1	GP		is implicated in					mRNA	NucleicAcid	export of			NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_10_1188_s_77	15905407	A number of previous studies have implicated Mlp1 in mRNA export; Mlp1 is known to bind to the hnRNP and mRNA export factor, Nab2 (Green et al. 2003 ).	bind
51263	2	11575	5	NULL	NULL	NULL	NULL	Mlp1	GP		bind					hnRNP	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_10_1188_s_77	15905407	A number of previous studies have implicated Mlp1 in mRNA export; Mlp1 is known to bind to the hnRNP and mRNA export factor, Nab2 (Green et al. 2003 ).	bind
51264	3	11575	5	NULL	NULL	NULL	NULL	Mlp1	GP		bind					Nab2	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_10_1188_s_77	15905407	A number of previous studies have implicated Mlp1 in mRNA export; Mlp1 is known to bind to the hnRNP and mRNA export factor, Nab2 (Green et al. 2003 ).	bind
51265	4	11575	5	NULL	NULL	NULL	NULL	Nab2	GP		is a type of					mRNA export factor	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_19_10_1188_s_77	15905407	A number of previous studies have implicated Mlp1 in mRNA export; Mlp1 is known to bind to the hnRNP and mRNA export factor, Nab2 (Green et al. 2003 ).	bind
50617	1	11575	6	NULL	NULL	0	NULL	Mlp1	NULL		bind	NULL				hnRNP	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_10_1188_s_77	15905407	A number of previous studies have implicated Mlp1 in mRNA export; Mlp1 is known to bind to the hnRNP and mRNA export factor, Nab2 (Green et al. 2003 ).	bind
50618	2	11575	6	NULL	NULL	0	NULL	Mlp1	NULL		bind	NULL				Nab2	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_10_1188_s_77	15905407	A number of previous studies have implicated Mlp1 in mRNA export; Mlp1 is known to bind to the hnRNP and mRNA export factor, Nab2 (Green et al. 2003 ).	bind
50619	3	11575	6	NULL	NULL	0	NULL	Nab2	NULL		is a type of	NULL				mRNA export factor	NULL				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_10_1188_s_77	15905407	A number of previous studies have implicated Mlp1 in mRNA export; Mlp1 is known to bind to the hnRNP and mRNA export factor, Nab2 (Green et al. 2003 ).	bind
58815	4	11575	6	10	NULL	0	NULL	Mlp1			is implicated in					mRNA		export of			NULL		0	NULL	NULL	NULL	gw70_genesdev_19_10_1188_s_77	15905407	A number of previous studies have implicated Mlp1 in mRNA export; Mlp1 is known to bind to the hnRNP and mRNA export factor, Nab2 (Green et al. 2003 ).	bind
51266	1	11576	5	NULL	NULL	NULL	NULL	MIBP1 homolog	GP	rat	bind		specifically						NF-kappaB-like motifs		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3736_s_211	10207097	A number of previous studies have shown that the rat MIBP1 homolog, the human MBP2 homolog, the partial MIBP1 clone AGIE-BP1, and the sequence-related transcription factor PRDII-BP1 bind specifically to NF-kappaB-like motifs with the consensus GGG N(4-5)CC ( 6,  11,  14,  17,  22).	bind
51267	2	11576	5	NULL	NULL	NULL	NULL	NF-kappaB-like motifs	GP		contains							consensus	GGG N(4-5)CC		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3736_s_211	10207097	A number of previous studies have shown that the rat MIBP1 homolog, the human MBP2 homolog, the partial MIBP1 clone AGIE-BP1, and the sequence-related transcription factor PRDII-BP1 bind specifically to NF-kappaB-like motifs with the consensus GGG N(4-5)CC ( 6,  11,  14,  17,  22).	bind
51268	3	11576	5	NULL	NULL	NULL	NULL	MBP2 homolog	GP	human	bind		specifically						NF-kappaB-like motifs		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3736_s_211	10207097	A number of previous studies have shown that the rat MIBP1 homolog, the human MBP2 homolog, the partial MIBP1 clone AGIE-BP1, and the sequence-related transcription factor PRDII-BP1 bind specifically to NF-kappaB-like motifs with the consensus GGG N(4-5)CC ( 6,  11,  14,  17,  22).	bind
51269	4	11576	5	NULL	NULL	NULL	NULL	AGIE-BP1	NucleicAcid		is a type of					partial MIBP1 clone	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3736_s_211	10207097	A number of previous studies have shown that the rat MIBP1 homolog, the human MBP2 homolog, the partial MIBP1 clone AGIE-BP1, and the sequence-related transcription factor PRDII-BP1 bind specifically to NF-kappaB-like motifs with the consensus GGG N(4-5)CC ( 6,  11,  14,  17,  22).	bind
51270	5	11576	5	NULL	NULL	NULL	NULL	AGIE-BP1	NucleicAcid		bind								NF-kappaB-like motifs		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3736_s_211	10207097	A number of previous studies have shown that the rat MIBP1 homolog, the human MBP2 homolog, the partial MIBP1 clone AGIE-BP1, and the sequence-related transcription factor PRDII-BP1 bind specifically to NF-kappaB-like motifs with the consensus GGG N(4-5)CC ( 6,  11,  14,  17,  22).	bind
51271	6	11576	5	NULL	NULL	NULL	NULL	PRDII-BP1	GP		is a type of					transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3736_s_211	10207097	A number of previous studies have shown that the rat MIBP1 homolog, the human MBP2 homolog, the partial MIBP1 clone AGIE-BP1, and the sequence-related transcription factor PRDII-BP1 bind specifically to NF-kappaB-like motifs with the consensus GGG N(4-5)CC ( 6,  11,  14,  17,  22).	bind
51272	7	11576	5	NULL	NULL	NULL	NULL	PRDII-BP1	GP		bind		specifically						NF-kappaB-like motifs		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3736_s_211	10207097	A number of previous studies have shown that the rat MIBP1 homolog, the human MBP2 homolog, the partial MIBP1 clone AGIE-BP1, and the sequence-related transcription factor PRDII-BP1 bind specifically to NF-kappaB-like motifs with the consensus GGG N(4-5)CC ( 6,  11,  14,  17,  22).	bind
50620	1	11576	6	NULL	NULL	0	NULL	MIBP1 homolog	NULL	rat	bind	NULL	specifically				NULL			NF-kappaB-like motifs	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3736_s_211	10207097	A number of previous studies have shown that the rat MIBP1 homolog, the human MBP2 homolog, the partial MIBP1 clone AGIE-BP1, and the sequence-related transcription factor PRDII-BP1 bind specifically to NF-kappaB-like motifs with the consensus GGG N(4-5)CC ( 6,  11,  14,  17,  22).	bind
50621	2	11576	6	10	NULL	0	NULL	NF-kappaB-like motifs			contains					GGG N(4-5)CC 		consensus			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3736_s_211	10207097	A number of previous studies have shown that the rat MIBP1 homolog, the human MBP2 homolog, the partial MIBP1 clone AGIE-BP1, and the sequence-related transcription factor PRDII-BP1 bind specifically to NF-kappaB-like motifs with the consensus GGG N(4-5)CC ( 6,  11,  14,  17,  22).	bind
50622	3	11576	6	10	NULL	0	NULL	MBP2 homolog		human	bind		specifically							NF-kappaB-like motifs	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3736_s_211	10207097	A number of previous studies have shown that the rat MIBP1 homolog, the human MBP2 homolog, the partial MIBP1 clone AGIE-BP1, and the sequence-related transcription factor PRDII-BP1 bind specifically to NF-kappaB-like motifs with the consensus GGG N(4-5)CC ( 6,  11,  14,  17,  22).	bind
50623	4	11576	6	NULL	NULL	0	NULL	PRDII-BP1	NULL		bind	NULL	specifically				NULL			NF-kappaB-like motifs	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3736_s_211	10207097	A number of previous studies have shown that the rat MIBP1 homolog, the human MBP2 homolog, the partial MIBP1 clone AGIE-BP1, and the sequence-related transcription factor PRDII-BP1 bind specifically to NF-kappaB-like motifs with the consensus GGG N(4-5)CC ( 6,  11,  14,  17,  22).	bind
50624	5	11576	6	NULL	NULL	0	NULL	PRDII-BP1	NULL		is a type of	NULL				transcription factor	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3736_s_211	10207097	A number of previous studies have shown that the rat MIBP1 homolog, the human MBP2 homolog, the partial MIBP1 clone AGIE-BP1, and the sequence-related transcription factor PRDII-BP1 bind specifically to NF-kappaB-like motifs with the consensus GGG N(4-5)CC ( 6,  11,  14,  17,  22).	bind
50625	6	11576	6	NULL	NULL	0	NULL	AGIE-BP1	NULL		bind	NULL					NULL			NF-kappaB-like motifs	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3736_s_211	10207097	A number of previous studies have shown that the rat MIBP1 homolog, the human MBP2 homolog, the partial MIBP1 clone AGIE-BP1, and the sequence-related transcription factor PRDII-BP1 bind specifically to NF-kappaB-like motifs with the consensus GGG N(4-5)CC ( 6,  11,  14,  17,  22).	bind
50626	7	11576	6	10	NULL	0	NULL	AGIE-BP1			is a type of					partial MIBP1 clone					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3736_s_211	10207097	A number of previous studies have shown that the rat MIBP1 homolog, the human MBP2 homolog, the partial MIBP1 clone AGIE-BP1, and the sequence-related transcription factor PRDII-BP1 bind specifically to NF-kappaB-like motifs with the consensus GGG N(4-5)CC ( 6,  11,  14,  17,  22).	bind
51281	1	11577	5	NULL	NULL	NULL	NULL	GM1	Chemical		is a type of					ganglioside	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_5_3204_s_11	12446685	A number of protein toxins utilize plasma membrane lipids as their receptors;  e.g. cholera toxin binds ganglioside GM1  ( 1), shiga toxin recognizes glycolipid Gb3  ( 2), and lysenin shows high affinity for sphingomyelin  ( 3).	bind
51282	2	11577	5	NULL	NULL	NULL	NULL	GM1	Chemical		is a type of					plasma membrane lipid	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_5_3204_s_11	12446685	A number of protein toxins utilize plasma membrane lipids as their receptors;  e.g. cholera toxin binds ganglioside GM1  ( 1), shiga toxin recognizes glycolipid Gb3  ( 2), and lysenin shows high affinity for sphingomyelin  ( 3).	bind
51283	3	11577	5	NULL	NULL	NULL	NULL	cholera toxin	GP		bind					GM1	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_5_3204_s_11	12446685	A number of protein toxins utilize plasma membrane lipids as their receptors;  e.g. cholera toxin binds ganglioside GM1  ( 1), shiga toxin recognizes glycolipid Gb3  ( 2), and lysenin shows high affinity for sphingomyelin  ( 3).	bind
51284	4	11577	5	NULL	NULL	NULL	NULL	Gb3	Chemical		is a type of					glycolipid	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_5_3204_s_11	12446685	A number of protein toxins utilize plasma membrane lipids as their receptors;  e.g. cholera toxin binds ganglioside GM1  ( 1), shiga toxin recognizes glycolipid Gb3  ( 2), and lysenin shows high affinity for sphingomyelin  ( 3).	bind
51285	5	11577	5	NULL	NULL	NULL	NULL	Gb3	Chemical		is a type of					plasma membrane lipid	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_5_3204_s_11	12446685	A number of protein toxins utilize plasma membrane lipids as their receptors;  e.g. cholera toxin binds ganglioside GM1  ( 1), shiga toxin recognizes glycolipid Gb3  ( 2), and lysenin shows high affinity for sphingomyelin  ( 3).	bind
51286	6	11577	5	NULL	NULL	NULL	NULL	shiga toxin	GP		recognizes					Gb3	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_5_3204_s_11	12446685	A number of protein toxins utilize plasma membrane lipids as their receptors;  e.g. cholera toxin binds ganglioside GM1  ( 1), shiga toxin recognizes glycolipid Gb3  ( 2), and lysenin shows high affinity for sphingomyelin  ( 3).	bind
51287	7	11577	5	NULL	NULL	NULL	NULL	sphingomyelin	Chemical		is a type of					plasma membrane lipid	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_5_3204_s_11	12446685	A number of protein toxins utilize plasma membrane lipids as their receptors;  e.g. cholera toxin binds ganglioside GM1  ( 1), shiga toxin recognizes glycolipid Gb3  ( 2), and lysenin shows high affinity for sphingomyelin  ( 3).	bind
51288	8	11577	5	NULL	NULL	NULL	NULL	lysenin	GP		affinity for		high			sphingomyelin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_5_3204_s_11	12446685	A number of protein toxins utilize plasma membrane lipids as their receptors;  e.g. cholera toxin binds ganglioside GM1  ( 1), shiga toxin recognizes glycolipid Gb3  ( 2), and lysenin shows high affinity for sphingomyelin  ( 3).	bind
50627	1	11577	6	NULL	NULL	0	NULL	cholera toxin	NULL		bind	NULL				GM1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_5_3204_s_11	12446685	A number of protein toxins utilize plasma membrane lipids as their receptors;  e.g. cholera toxin binds ganglioside GM1  ( 1), shiga toxin recognizes glycolipid Gb3  ( 2), and lysenin shows high affinity for sphingomyelin  ( 3).	bind
50628	2	11577	6	NULL	NULL	0	NULL	GM1	NULL		is a type of	NULL				ganglioside	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_5_3204_s_11	12446685	A number of protein toxins utilize plasma membrane lipids as their receptors;  e.g. cholera toxin binds ganglioside GM1  ( 1), shiga toxin recognizes glycolipid Gb3  ( 2), and lysenin shows high affinity for sphingomyelin  ( 3).	bind
50629	3	11577	6	10	NULL	0	NULL	shiga toxin			recognizes					Gb3					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_5_3204_s_11	12446685	A number of protein toxins utilize plasma membrane lipids as their receptors;  e.g. cholera toxin binds ganglioside GM1  ( 1), shiga toxin recognizes glycolipid Gb3  ( 2), and lysenin shows high affinity for sphingomyelin  ( 3).	bind
50630	4	11577	6	NULL	NULL	0	NULL	Gb3	NULL		is a type of	NULL				glycolipid	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_5_3204_s_11	12446685	A number of protein toxins utilize plasma membrane lipids as their receptors;  e.g. cholera toxin binds ganglioside GM1  ( 1), shiga toxin recognizes glycolipid Gb3  ( 2), and lysenin shows high affinity for sphingomyelin  ( 3).	bind
50631	5	11577	6	NULL	NULL	0	NULL	lysenin	NULL		has affinity for	NULL	high			sphingomyelin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_5_3204_s_11	12446685	A number of protein toxins utilize plasma membrane lipids as their receptors;  e.g. cholera toxin binds ganglioside GM1  ( 1), shiga toxin recognizes glycolipid Gb3  ( 2), and lysenin shows high affinity for sphingomyelin  ( 3).	bind
50632	6	11577	6	NULL	NULL	0	NULL	ganglioside	NULL		is a type of	NULL				plasma membrane lipids	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_5_3204_s_11	12446685	A number of protein toxins utilize plasma membrane lipids as their receptors;  e.g. cholera toxin binds ganglioside GM1  ( 1), shiga toxin recognizes glycolipid Gb3  ( 2), and lysenin shows high affinity for sphingomyelin  ( 3).	bind
50633	7	11577	6	NULL	NULL	0	NULL	glycolipid	NULL		is a type of	NULL				plasma membrane lipid	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_5_3204_s_11	12446685	A number of protein toxins utilize plasma membrane lipids as their receptors;  e.g. cholera toxin binds ganglioside GM1  ( 1), shiga toxin recognizes glycolipid Gb3  ( 2), and lysenin shows high affinity for sphingomyelin  ( 3).	bind
50634	8	11577	6	NULL	NULL	0	NULL	sphingomyelin	NULL		is a type of	NULL				plasma membrane lipid	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_5_3204_s_11	12446685	A number of protein toxins utilize plasma membrane lipids as their receptors;  e.g. cholera toxin binds ganglioside GM1  ( 1), shiga toxin recognizes glycolipid Gb3  ( 2), and lysenin shows high affinity for sphingomyelin  ( 3).	bind
51289	1	11579	5	NULL	NULL	NULL	NULL	Rho	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_7_1_12_s_264	8999996	A number of proteins have recently been identified that specifically interact with the GTP-bound form of Rho (reviewed in  [30]  ).	bind
50635	1	11579	6	NULL	NULL	0	NULL	GTP	NULL		bind	NULL				Rho	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_7_1_12_s_264	8999996	A number of proteins have recently been identified that specifically interact with the GTP-bound form of Rho (reviewed in  [30]  ).	bind
51290	1	11580	5	NULL	NULL	NULL	NULL	PRRs	GP		is present in					insects	Organism				NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_28_1_101_s_147	14975532	A number of PRRs are present in insects  ( Table 2) and include: the C-type lectins which bind bacterial LPS, the peptidoglycan recognition  protein which is expressed in the fat body, haemocytes and epithelial cells and the   -1,3 glucan binding protein which recognises fungal glucan and activates the ProPO-AS  pathway.	bind
51291	2	11580	5	NULL	NULL	NULL	NULL	C-type lectins	Chemical		is a type of					PRR	GP				NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_28_1_101_s_147	14975532	A number of PRRs are present in insects  ( Table 2) and include: the C-type lectins which bind bacterial LPS, the peptidoglycan recognition  protein which is expressed in the fat body, haemocytes and epithelial cells and the   -1,3 glucan binding protein which recognises fungal glucan and activates the ProPO-AS  pathway.	bind
51292	3	11580	5	NULL	NULL	NULL	NULL	C-type lectins	GP		bind					LPS	GP	bacterial			NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_28_1_101_s_147	14975532	A number of PRRs are present in insects  ( Table 2) and include: the C-type lectins which bind bacterial LPS, the peptidoglycan recognition  protein which is expressed in the fat body, haemocytes and epithelial cells and the   -1,3 glucan binding protein which recognises fungal glucan and activates the ProPO-AS  pathway.	bind
51293	4	11580	5	NULL	NULL	NULL	NULL	LPS	GP		is a type of					peptidoglycan recognition protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_28_1_101_s_147	14975532	A number of PRRs are present in insects  ( Table 2) and include: the C-type lectins which bind bacterial LPS, the peptidoglycan recognition  protein which is expressed in the fat body, haemocytes and epithelial cells and the   -1,3 glucan binding protein which recognises fungal glucan and activates the ProPO-AS  pathway.	bind
51294	5	11580	5	NULL	NULL	NULL	NULL	LPS	GP	bacterial	is expressed in					fat body	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_28_1_101_s_147	14975532	A number of PRRs are present in insects  ( Table 2) and include: the C-type lectins which bind bacterial LPS, the peptidoglycan recognition  protein which is expressed in the fat body, haemocytes and epithelial cells and the   -1,3 glucan binding protein which recognises fungal glucan and activates the ProPO-AS  pathway.	bind
51295	6	11580	5	NULL	NULL	NULL	NULL	LPS	GP	bacterial	is expressed in					haemocytes	Cell				NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_28_1_101_s_147	14975532	A number of PRRs are present in insects  ( Table 2) and include: the C-type lectins which bind bacterial LPS, the peptidoglycan recognition  protein which is expressed in the fat body, haemocytes and epithelial cells and the   -1,3 glucan binding protein which recognises fungal glucan and activates the ProPO-AS  pathway.	bind
51296	7	11580	5	NULL	NULL	NULL	NULL	LPS	GP	bacterial	is expressed in					epithelial cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_28_1_101_s_147	14975532	A number of PRRs are present in insects  ( Table 2) and include: the C-type lectins which bind bacterial LPS, the peptidoglycan recognition  protein which is expressed in the fat body, haemocytes and epithelial cells and the   -1,3 glucan binding protein which recognises fungal glucan and activates the ProPO-AS  pathway.	bind
51297	8	11580	5	NULL	NULL	NULL	NULL	-1,3 glucan binding protein	GP		is a type of					PRR	GP				NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_28_1_101_s_147	14975532	A number of PRRs are present in insects  ( Table 2) and include: the C-type lectins which bind bacterial LPS, the peptidoglycan recognition  protein which is expressed in the fat body, haemocytes and epithelial cells and the   -1,3 glucan binding protein which recognises fungal glucan and activates the ProPO-AS  pathway.	bind
51298	9	11580	5	NULL	NULL	NULL	NULL	-1,3 glucan binding protein	GP		recognizes					glucan	Chemical	fungal			NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_28_1_101_s_147	14975532	A number of PRRs are present in insects  ( Table 2) and include: the C-type lectins which bind bacterial LPS, the peptidoglycan recognition  protein which is expressed in the fat body, haemocytes and epithelial cells and the   -1,3 glucan binding protein which recognises fungal glucan and activates the ProPO-AS  pathway.	bind
51299	10	11580	5	NULL	NULL	NULL	NULL	-1,3 glucan binding protein	GP		activates					ProPO-AS pathway	Process				NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_28_1_101_s_147	14975532	A number of PRRs are present in insects  ( Table 2) and include: the C-type lectins which bind bacterial LPS, the peptidoglycan recognition  protein which is expressed in the fat body, haemocytes and epithelial cells and the   -1,3 glucan binding protein which recognises fungal glucan and activates the ProPO-AS  pathway.	bind
50636	1	11580	6	NULL	NULL	0	NULL	C-type lectins	NULL		bind	NULL				LPS	NULL	bacterial			NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_28_1_101_s_147	14975532	A number of PRRs are present in insects  ( Table 2) and include: the C-type lectins which bind bacterial LPS, the peptidoglycan recognition  protein which is expressed in the fat body, haemocytes and epithelial cells and the   -1,3 glucan binding protein which recognises fungal glucan and activates the ProPO-AS  pathway.	bind
50637	2	11580	6	NULL	NULL	0	NULL	peptidoglycan recognition protein	NULL		is expressed in	NULL				fat body	NULL				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_28_1_101_s_147	14975532	A number of PRRs are present in insects  ( Table 2) and include: the C-type lectins which bind bacterial LPS, the peptidoglycan recognition  protein which is expressed in the fat body, haemocytes and epithelial cells and the   -1,3 glucan binding protein which recognises fungal glucan and activates the ProPO-AS  pathway.	bind
50638	3	11580	6	NULL	NULL	0	NULL	peptidoglycan recognition protein	NULL		is expressed in	NULL				haemocytes	NULL				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_28_1_101_s_147	14975532	A number of PRRs are present in insects  ( Table 2) and include: the C-type lectins which bind bacterial LPS, the peptidoglycan recognition  protein which is expressed in the fat body, haemocytes and epithelial cells and the   -1,3 glucan binding protein which recognises fungal glucan and activates the ProPO-AS  pathway.	bind
50639	4	11580	6	NULL	NULL	0	NULL	peptidoglycan recognition protein	NULL		is expressed in	NULL				epithelial cells	NULL				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_28_1_101_s_147	14975532	A number of PRRs are present in insects  ( Table 2) and include: the C-type lectins which bind bacterial LPS, the peptidoglycan recognition  protein which is expressed in the fat body, haemocytes and epithelial cells and the   -1,3 glucan binding protein which recognises fungal glucan and activates the ProPO-AS  pathway.	bind
50640	5	11580	6	NULL	NULL	0	NULL	1,3 glucan binding protein	NULL		recognizes	NULL				fungal glucan	NULL				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_28_1_101_s_147	14975532	A number of PRRs are present in insects  ( Table 2) and include: the C-type lectins which bind bacterial LPS, the peptidoglycan recognition  protein which is expressed in the fat body, haemocytes and epithelial cells and the   -1,3 glucan binding protein which recognises fungal glucan and activates the ProPO-AS  pathway.	bind
50641	6	11580	6	NULL	NULL	0	NULL	1,3 glucan binding protein	NULL		activates	NULL				ProPO-AS pathway	NULL				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_28_1_101_s_147	14975532	A number of PRRs are present in insects  ( Table 2) and include: the C-type lectins which bind bacterial LPS, the peptidoglycan recognition  protein which is expressed in the fat body, haemocytes and epithelial cells and the   -1,3 glucan binding protein which recognises fungal glucan and activates the ProPO-AS  pathway.	bind
50642	7	11580	6	NULL	NULL	0	NULL	C-type lectins	NULL		is a type of	NULL				PRR	NULL				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_28_1_101_s_147	14975532	A number of PRRs are present in insects  ( Table 2) and include: the C-type lectins which bind bacterial LPS, the peptidoglycan recognition  protein which is expressed in the fat body, haemocytes and epithelial cells and the   -1,3 glucan binding protein which recognises fungal glucan and activates the ProPO-AS  pathway.	bind
50643	8	11580	6	10	NULL	0	NULL	LPS			is a type of					peptidoglycan recognition protein					NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_28_1_101_s_147	14975532	A number of PRRs are present in insects  ( Table 2) and include: the C-type lectins which bind bacterial LPS, the peptidoglycan recognition  protein which is expressed in the fat body, haemocytes and epithelial cells and the   -1,3 glucan binding protein which recognises fungal glucan and activates the ProPO-AS  pathway.	bind
50644	9	11580	6	NULL	NULL	0	NULL	1,3 glucan binding protein	NULL		is a type of	NULL				PRR	NULL				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_28_1_101_s_147	14975532	A number of PRRs are present in insects  ( Table 2) and include: the C-type lectins which bind bacterial LPS, the peptidoglycan recognition  protein which is expressed in the fat body, haemocytes and epithelial cells and the   -1,3 glucan binding protein which recognises fungal glucan and activates the ProPO-AS  pathway.	bind
50645	10	11580	6	NULL	NULL	0	NULL	PRR	NULL		is present in	NULL				insects	NULL				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_28_1_101_s_147	14975532	A number of PRRs are present in insects  ( Table 2) and include: the C-type lectins which bind bacterial LPS, the peptidoglycan recognition  protein which is expressed in the fat body, haemocytes and epithelial cells and the   -1,3 glucan binding protein which recognises fungal glucan and activates the ProPO-AS  pathway.	bind
51300	1	11581	5	NULL	NULL	0	NULL		NULL		bind	NULL		PTB domains			NULL	phosphorylated	NP XY motifs		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_22_19119_s_262	11259429	A number of PTB domains have been identified, some of which bind phosphorylated NP XY motifs, whereas others bind unphosphorylated NP XY motifs ( 15).	bind
51301	2	11581	5	NULL	NULL	0	NULL		NULL		bind	NULL		PTB domains			NULL	unphosphorylated	NP XY motifs		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_22_19119_s_262	11259429	A number of PTB domains have been identified, some of which bind phosphorylated NP XY motifs, whereas others bind unphosphorylated NP XY motifs ( 15).	bind
50646	1	11581	6	NULL	NULL	0	NULL		NULL		bind	NULL		PTB domain			NULL	phosphorylated	NP XY motifs		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_22_19119_s_262	11259429	A number of PTB domains have been identified, some of which bind phosphorylated NP XY motifs, whereas others bind unphosphorylated NP XY motifs ( 15).	bind
50647	2	11581	6	NULL	NULL	0	NULL		NULL		bind	NULL		PTB domain			NULL	unphosphorylated	NP XY motifs		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_22_19119_s_262	11259429	A number of PTB domains have been identified, some of which bind phosphorylated NP XY motifs, whereas others bind unphosphorylated NP XY motifs ( 15).	bind
51302	1	11582	5	NULL	NULL	0	NULL		NULL	putative	is present in	NULL			GATA binding sites	CNS-1	NULL				NULL		0	NULL	NULL	NULL	gw70_jclininvest_116_5_1327_s_131	16628252	A number of putative GATA and Ikaros binding sites are present within both CNS-1 and VAE (Figure  5A).	bind
51303	2	11582	5	NULL	NULL	0	NULL		NULL	putative	is present in	NULL			GATA binding sites	VAE	NULL				NULL		0	NULL	NULL	NULL	gw70_jclininvest_116_5_1327_s_131	16628252	A number of putative GATA and Ikaros binding sites are present within both CNS-1 and VAE (Figure  5A).	bind
51304	3	11582	5	NULL	NULL	0	NULL		NULL	putative	is present in	NULL			Ikaros binding site	CNS-1	NULL				NULL		0	NULL	NULL	NULL	gw70_jclininvest_116_5_1327_s_131	16628252	A number of putative GATA and Ikaros binding sites are present within both CNS-1 and VAE (Figure  5A).	bind
51305	4	11582	5	NULL	NULL	0	NULL		NULL	putative	is present in	NULL			Ikaros binding site	VAE	NULL				NULL		0	NULL	NULL	NULL	gw70_jclininvest_116_5_1327_s_131	16628252	A number of putative GATA and Ikaros binding sites are present within both CNS-1 and VAE (Figure  5A).	bind
50648	1	11582	6	NULL	NULL	0	NULL	CNS-1	NULL		contains	NULL					NULL	putative		GATA binding sites	NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_5_1327_s_131	16628252	A number of putative GATA and Ikaros binding sites are present within both CNS-1 and VAE (Figure  5A).	bind
50649	2	11582	6	NULL	NULL	0	NULL	CNS-1	NULL		contains	NULL					NULL	putative		Ikaros binding site	NULL		0	NULL	NULL	NULL	gw70_jclininvest_116_5_1327_s_131	16628252	A number of putative GATA and Ikaros binding sites are present within both CNS-1 and VAE (Figure  5A).	bind
50650	3	11582	6	NULL	NULL	0	NULL	VAE	NULL		contains	NULL					NULL	putative		GATA binding site	NULL		0	NULL	NULL	NULL	gw70_jclininvest_116_5_1327_s_131	16628252	A number of putative GATA and Ikaros binding sites are present within both CNS-1 and VAE (Figure  5A).	bind
50651	4	11582	6	NULL	NULL	0	NULL	VAE	NULL		contains	NULL					NULL	putative		Ikaros binding site	NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_116_5_1327_s_131	16628252	A number of putative GATA and Ikaros binding sites are present within both CNS-1 and VAE (Figure  5A).	bind
51306	1	11583	5	NULL	NULL	NULL	NULL	Rac	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_29_17991_s_10	9660749	A number of Rac targets have been identified to date, based on their ability to interact preferentially with the GTP-bound form of Rac.	bind
50502	1	11583	6	NULL	NULL	0	NULL	Rac	NULL		bind	NULL				GTP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_29_17991_s_10	9660749	A number of Rac targets have been identified to date, based on their ability to interact preferentially with the GTP-bound form of Rac.	bind
51307	1	11585	5	NULL	NULL	NULL	NULL	c-Myc	GP	ectopic expression of	induce					hTERT	GP	expression of			NULL	human cells	NULL	NULL	NULL	NULL	gw60_pnas_98_7_3826_s_183	11274400	A number of recent observations support the identification of the  hTERT gene as a c-Myc target: ( i) ectopic expression of c-Myc induced  hTERT expression and activated telomerase activity in human cells ( 27); ( ii) the specific Myc binding motifs, E-boxes, are present in the  hTERT promoter, and the activity of the promoter is significantly increased by transient expression of c-Myc ( 7,  28,  29,  39); ( iii) ectopic expression of the Mad1 protein results in repression of  hTERT expression ( 30,  31); and ( iv)  in vivo interaction between N-Myc and the  hTERT promoter was recently observed in a neuroblastoma cell line transfected with N- myc ( 40).	bind
51308	2	11585	5	NULL	NULL	NULL	NULL	hTERT	GP		contains				promoter					Myc binding motifs	NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_7_3826_s_183	11274400	A number of recent observations support the identification of the  hTERT gene as a c-Myc target: ( i) ectopic expression of c-Myc induced  hTERT expression and activated telomerase activity in human cells ( 27); ( ii) the specific Myc binding motifs, E-boxes, are present in the  hTERT promoter, and the activity of the promoter is significantly increased by transient expression of c-Myc ( 7,  28,  29,  39); ( iii) ectopic expression of the Mad1 protein results in repression of  hTERT expression ( 30,  31); and ( iv)  in vivo interaction between N-Myc and the  hTERT promoter was recently observed in a neuroblastoma cell line transfected with N- myc ( 40).	bind
51309	3	11585	5	NULL	NULL	NULL	NULL	hTERT	GP		contains				promoter					E-boxes	NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_7_3826_s_183	11274400	A number of recent observations support the identification of the  hTERT gene as a c-Myc target: ( i) ectopic expression of c-Myc induced  hTERT expression and activated telomerase activity in human cells ( 27); ( ii) the specific Myc binding motifs, E-boxes, are present in the  hTERT promoter, and the activity of the promoter is significantly increased by transient expression of c-Myc ( 7,  28,  29,  39); ( iii) ectopic expression of the Mad1 protein results in repression of  hTERT expression ( 30,  31); and ( iv)  in vivo interaction between N-Myc and the  hTERT promoter was recently observed in a neuroblastoma cell line transfected with N- myc ( 40).	bind
51310	4	11585	5	NULL	NULL	NULL	NULL	c-Myc	GP	transient expression of	increase		significantly			hTERT	GP	activity of		promoter	NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_7_3826_s_183	11274400	A number of recent observations support the identification of the  hTERT gene as a c-Myc target: ( i) ectopic expression of c-Myc induced  hTERT expression and activated telomerase activity in human cells ( 27); ( ii) the specific Myc binding motifs, E-boxes, are present in the  hTERT promoter, and the activity of the promoter is significantly increased by transient expression of c-Myc ( 7,  28,  29,  39); ( iii) ectopic expression of the Mad1 protein results in repression of  hTERT expression ( 30,  31); and ( iv)  in vivo interaction between N-Myc and the  hTERT promoter was recently observed in a neuroblastoma cell line transfected with N- myc ( 40).	bind
51311	5	11585	5	NULL	NULL	NULL	NULL	Mad1 protein	GP	ectopic expression of	repress					hTERT	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_7_3826_s_183	11274400	A number of recent observations support the identification of the  hTERT gene as a c-Myc target: ( i) ectopic expression of c-Myc induced  hTERT expression and activated telomerase activity in human cells ( 27); ( ii) the specific Myc binding motifs, E-boxes, are present in the  hTERT promoter, and the activity of the promoter is significantly increased by transient expression of c-Myc ( 7,  28,  29,  39); ( iii) ectopic expression of the Mad1 protein results in repression of  hTERT expression ( 30,  31); and ( iv)  in vivo interaction between N-Myc and the  hTERT promoter was recently observed in a neuroblastoma cell line transfected with N- myc ( 40).	bind
51312	6	11585	5	NULL	NULL	NULL	NULL	N-Myc	GP		interacts with					hTERT	GP			promoter	NULL	in vivo in neuroblastoma cell line transfected with N- myc	NULL	NULL	NULL	NULL	gw60_pnas_98_7_3826_s_183	11274400	A number of recent observations support the identification of the  hTERT gene as a c-Myc target: ( i) ectopic expression of c-Myc induced  hTERT expression and activated telomerase activity in human cells ( 27); ( ii) the specific Myc binding motifs, E-boxes, are present in the  hTERT promoter, and the activity of the promoter is significantly increased by transient expression of c-Myc ( 7,  28,  29,  39); ( iii) ectopic expression of the Mad1 protein results in repression of  hTERT expression ( 30,  31); and ( iv)  in vivo interaction between N-Myc and the  hTERT promoter was recently observed in a neuroblastoma cell line transfected with N- myc ( 40).	bind
51313	7	11585	5	NULL	NULL	NULL	NULL	c-Myc	GP	ectopic expression of	activates					telomerase	GP	activity of			NULL	human cells	NULL	NULL	NULL	NULL	gw60_pnas_98_7_3826_s_183	11274400	A number of recent observations support the identification of the  hTERT gene as a c-Myc target: ( i) ectopic expression of c-Myc induced  hTERT expression and activated telomerase activity in human cells ( 27); ( ii) the specific Myc binding motifs, E-boxes, are present in the  hTERT promoter, and the activity of the promoter is significantly increased by transient expression of c-Myc ( 7,  28,  29,  39); ( iii) ectopic expression of the Mad1 protein results in repression of  hTERT expression ( 30,  31); and ( iv)  in vivo interaction between N-Myc and the  hTERT promoter was recently observed in a neuroblastoma cell line transfected with N- myc ( 40).	bind
50652	1	11585	6	10	NULL	0	NULL	N-Myc			interacts with					hTERT				promoter	NULL	in vivo in neuroblastoma cell line transfected with N- myc	NULL	NULL	NULL	NULL	gw60_pnas_98_7_3826_s_183	11274400	A number of recent observations support the identification of the  hTERT gene as a c-Myc target: ( i) ectopic expression of c-Myc induced  hTERT expression and activated telomerase activity in human cells ( 27); ( ii) the specific Myc binding motifs, E-boxes, are present in the  hTERT promoter, and the activity of the promoter is significantly increased by transient expression of c-Myc ( 7,  28,  29,  39); ( iii) ectopic expression of the Mad1 protein results in repression of  hTERT expression ( 30,  31); and ( iv)  in vivo interaction between N-Myc and the  hTERT promoter was recently observed in a neuroblastoma cell line transfected with N- myc ( 40).	bind
50653	2	11585	6	10	NULL	0	NULL	c-Myc		ectopic;; expression of	induces					hTERT		expression of 			NULL	human cells	NULL	NULL	NULL	NULL	gw60_pnas_98_7_3826_s_183	11274400	A number of recent observations support the identification of the  hTERT gene as a c-Myc target: ( i) ectopic expression of c-Myc induced  hTERT expression and activated telomerase activity in human cells ( 27); ( ii) the specific Myc binding motifs, E-boxes, are present in the  hTERT promoter, and the activity of the promoter is significantly increased by transient expression of c-Myc ( 7,  28,  29,  39); ( iii) ectopic expression of the Mad1 protein results in repression of  hTERT expression ( 30,  31); and ( iv)  in vivo interaction between N-Myc and the  hTERT promoter was recently observed in a neuroblastoma cell line transfected with N- myc ( 40).	bind
50654	3	11585	6	10	NULL	0	NULL	c-Myc		ectopic expression of	activates					telomerase 		activity of			NULL	human cells	NULL	NULL	NULL	NULL	gw60_pnas_98_7_3826_s_183	11274400	A number of recent observations support the identification of the  hTERT gene as a c-Myc target: ( i) ectopic expression of c-Myc induced  hTERT expression and activated telomerase activity in human cells ( 27); ( ii) the specific Myc binding motifs, E-boxes, are present in the  hTERT promoter, and the activity of the promoter is significantly increased by transient expression of c-Myc ( 7,  28,  29,  39); ( iii) ectopic expression of the Mad1 protein results in repression of  hTERT expression ( 30,  31); and ( iv)  in vivo interaction between N-Myc and the  hTERT promoter was recently observed in a neuroblastoma cell line transfected with N- myc ( 40).	bind
50655	4	11585	6	NULL	NULL	0	NULL	hTERT	NULL		contains	NULL					NULL	specific		Myc binding motif	NULL		0	NULL	NULL	NULL	gw60_pnas_98_7_3826_s_183	11274400	A number of recent observations support the identification of the  hTERT gene as a c-Myc target: ( i) ectopic expression of c-Myc induced  hTERT expression and activated telomerase activity in human cells ( 27); ( ii) the specific Myc binding motifs, E-boxes, are present in the  hTERT promoter, and the activity of the promoter is significantly increased by transient expression of c-Myc ( 7,  28,  29,  39); ( iii) ectopic expression of the Mad1 protein results in repression of  hTERT expression ( 30,  31); and ( iv)  in vivo interaction between N-Myc and the  hTERT promoter was recently observed in a neuroblastoma cell line transfected with N- myc ( 40).	bind
50656	5	11585	6	NULL	NULL	0	NULL	hTERT	NULL		contains	NULL					NULL			E-boxes	NULL		0	NULL	NULL	NULL	gw60_pnas_98_7_3826_s_183	11274400	A number of recent observations support the identification of the  hTERT gene as a c-Myc target: ( i) ectopic expression of c-Myc induced  hTERT expression and activated telomerase activity in human cells ( 27); ( ii) the specific Myc binding motifs, E-boxes, are present in the  hTERT promoter, and the activity of the promoter is significantly increased by transient expression of c-Myc ( 7,  28,  29,  39); ( iii) ectopic expression of the Mad1 protein results in repression of  hTERT expression ( 30,  31); and ( iv)  in vivo interaction between N-Myc and the  hTERT promoter was recently observed in a neuroblastoma cell line transfected with N- myc ( 40).	bind
50657	6	11585	6	NULL	NULL	0	NULL	hTERT	NULL	activity of	is increased 	NULL	significantly		promoter	c-Myc	NULL	transient expression of			NULL		0	NULL	NULL	NULL	gw60_pnas_98_7_3826_s_183	11274400	A number of recent observations support the identification of the  hTERT gene as a c-Myc target: ( i) ectopic expression of c-Myc induced  hTERT expression and activated telomerase activity in human cells ( 27); ( ii) the specific Myc binding motifs, E-boxes, are present in the  hTERT promoter, and the activity of the promoter is significantly increased by transient expression of c-Myc ( 7,  28,  29,  39); ( iii) ectopic expression of the Mad1 protein results in repression of  hTERT expression ( 30,  31); and ( iv)  in vivo interaction between N-Myc and the  hTERT promoter was recently observed in a neuroblastoma cell line transfected with N- myc ( 40).	bind
50658	7	11585	6	NULL	NULL	0	NULL	Mad1 protein	NULL	ectopic expression of	results in	NULL				hTERT	NULL	repression of			NULL		0	NULL	NULL	NULL	gw60_pnas_98_7_3826_s_183	11274400	A number of recent observations support the identification of the  hTERT gene as a c-Myc target: ( i) ectopic expression of c-Myc induced  hTERT expression and activated telomerase activity in human cells ( 27); ( ii) the specific Myc binding motifs, E-boxes, are present in the  hTERT promoter, and the activity of the promoter is significantly increased by transient expression of c-Myc ( 7,  28,  29,  39); ( iii) ectopic expression of the Mad1 protein results in repression of  hTERT expression ( 30,  31); and ( iv)  in vivo interaction between N-Myc and the  hTERT promoter was recently observed in a neuroblastoma cell line transfected with N- myc ( 40).	bind
51314	1	11586	5	NULL	NULL	NULL	NULL	Smad3	GP		bind		directly			DNA sequences	NucleicAcid	specific			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_19_3084_s_224	9765209	A number of recent reports show direct binding of Smad3 and Smad4 to specific DNA sequences, but these reports disagree on the consensus binding sequences (Yingling et al. 1997  ; Dennler et al. 1998  ; Vindevoghel et al. 1998  ; Zawel et al. 1998  ).	bind
51315	2	11586	5	NULL	NULL	NULL	NULL	Smad4	GP		bind		directly			DNA sequences	NucleicAcid	specific			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_19_3084_s_224	9765209	A number of recent reports show direct binding of Smad3 and Smad4 to specific DNA sequences, but these reports disagree on the consensus binding sequences (Yingling et al. 1997  ; Dennler et al. 1998  ; Vindevoghel et al. 1998  ; Zawel et al. 1998  ).	bind
50660	1	11586	6	NULL	NULL	0	NULL	Smad3	NULL		bind	NULL	directly			DNA sequencees	NULL	specific			NULL		0	NULL	NULL	NULL	gw60_genesdev_12_19_3084_s_224	9765209	A number of recent reports show direct binding of Smad3 and Smad4 to specific DNA sequences, but these reports disagree on the consensus binding sequences (Yingling et al. 1997  ; Dennler et al. 1998  ; Vindevoghel et al. 1998  ; Zawel et al. 1998  ).	bind
54218	2	11586	6	10	NULL	0	NULL	Smad4			bind		directly			DNA sequences		specific			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_19_3084_s_224	9765209	A number of recent reports show direct binding of Smad3 and Smad4 to specific DNA sequences, but these reports disagree on the consensus binding sequences (Yingling et al. 1997  ; Dennler et al. 1998  ; Vindevoghel et al. 1998  ; Zawel et al. 1998  ).	bind
51316	1	11587	5	NULL	NULL	NULL	NULL	importin	GP		is					cytosolic receptor	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_7_4197_s_336	9461616	A number of recent reports suggest that the nuclear targeting of most nuclear proteins is initiated by binding of cytosolic receptor (termed importin) to NLS.	bind
51317	2	11587	5	NULL	NULL	NULL	NULL	importin	GP		bind								NLS		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_7_4197_s_336	9461616	A number of recent reports suggest that the nuclear targeting of most nuclear proteins is initiated by binding of cytosolic receptor (termed importin) to NLS.	bind
51318	3	11587	5	NULL	NULL	NULL	NULL	statement 2	Process		initiates					nuclear proteins	GP	nuclear targeting of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_7_4197_s_336	9461616	A number of recent reports suggest that the nuclear targeting of most nuclear proteins is initiated by binding of cytosolic receptor (termed importin) to NLS.	bind
50661	1	11587	6	NULL	NULL	0	NULL	cytosolic receptor	NULL		bind	NULL				NLS	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_7_4197_s_336	9461616	A number of recent reports suggest that the nuclear targeting of most nuclear proteins is initiated by binding of cytosolic receptor (termed importin) to NLS.	bind
50662	2	11587	6	NULL	NULL	0	NULL	cytosolic receptor	NULL		is	NULL				importin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_7_4197_s_336	9461616	A number of recent reports suggest that the nuclear targeting of most nuclear proteins is initiated by binding of cytosolic receptor (termed importin) to NLS.	bind
58816	3	11587	6	10	NULL	0	NULL	statement 1			initiates					 nuclear proteins		nuclear targeting of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_7_4197_s_336	9461616	A number of recent reports suggest that the nuclear targeting of most nuclear proteins is initiated by binding of cytosolic receptor (termed importin) to NLS.	bind
51319	1	11588	5	NULL	NULL	NULL	NULL				is a type of				GATA binding site	regulatory site	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_33_29856_s_27	15941713	A number of regulatory sites have been identified including a GATA binding site ( ), Sp1 and Sp3 binding sites ( ,  ), as well as a NF-kappaB site ( ) shown to be involved in basal transcriptional activity.	bind
51320	2	11588	5	NULL	NULL	NULL	NULL				is a type of				Sp1 binding site	regulatory site	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_33_29856_s_27	15941713	A number of regulatory sites have been identified including a GATA binding site ( ), Sp1 and Sp3 binding sites ( ,  ), as well as a NF-kappaB site ( ) shown to be involved in basal transcriptional activity.	bind
51321	3	11588	5	NULL	NULL	NULL	NULL				is a type of				Sp3 binding site	regulatory site	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_33_29856_s_27	15941713	A number of regulatory sites have been identified including a GATA binding site ( ), Sp1 and Sp3 binding sites ( ,  ), as well as a NF-kappaB site ( ) shown to be involved in basal transcriptional activity.	bind
51322	4	11588	5	NULL	NULL	NULL	NULL				is a type of				NF-kappaB site	regulatory site	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_33_29856_s_27	15941713	A number of regulatory sites have been identified including a GATA binding site ( ), Sp1 and Sp3 binding sites ( ,  ), as well as a NF-kappaB site ( ) shown to be involved in basal transcriptional activity.	bind
51323	5	11588	5	NULL	NULL	NULL	NULL				is involved in				GATA binding site	transcriptional activity	Process	basal			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_33_29856_s_27	15941713	A number of regulatory sites have been identified including a GATA binding site ( ), Sp1 and Sp3 binding sites ( ,  ), as well as a NF-kappaB site ( ) shown to be involved in basal transcriptional activity.	bind
51326	6	11588	5	NULL	NULL	NULL	NULL				is involved in				Sp1 binding sites	transcriptional activity	Process	basal			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_33_29856_s_27	15941713	A number of regulatory sites have been identified including a GATA binding site ( ), Sp1 and Sp3 binding sites ( ,  ), as well as a NF-kappaB site ( ) shown to be involved in basal transcriptional activity.	bind
51327	7	11588	5	NULL	NULL	NULL	NULL				is involved in				Sp3 binding sites	transcriptional activity	Process	basal			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_33_29856_s_27	15941713	A number of regulatory sites have been identified including a GATA binding site ( ), Sp1 and Sp3 binding sites ( ,  ), as well as a NF-kappaB site ( ) shown to be involved in basal transcriptional activity.	bind
51328	8	11588	5	NULL	NULL	NULL	NULL				is involved in				NF-kappaB site	transcriptional activity	Process	basal			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_33_29856_s_27	15941713	A number of regulatory sites have been identified including a GATA binding site ( ), Sp1 and Sp3 binding sites ( ,  ), as well as a NF-kappaB site ( ) shown to be involved in basal transcriptional activity.	bind
50663	1	11588	6	NULL	NULL	0	NULL		NULL		is involved in	NULL			GATA binding site	transcriptional activity	NULL	basal			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_33_29856_s_27	15941713	A number of regulatory sites have been identified including a GATA binding site ( ), Sp1 and Sp3 binding sites ( ,  ), as well as a NF-kappaB site ( ) shown to be involved in basal transcriptional activity.	bind
50664	2	11588	6	NULL	NULL	0	NULL		NULL		is involved in	NULL			Sp1 binding site	transcriptional activity	NULL	basal			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_33_29856_s_27	15941713	A number of regulatory sites have been identified including a GATA binding site ( ), Sp1 and Sp3 binding sites ( ,  ), as well as a NF-kappaB site ( ) shown to be involved in basal transcriptional activity.	bind
50665	3	11588	6	NULL	NULL	0	NULL		NULL		is involved in	NULL			Sp3 binding site	transcriptional activity	NULL	basal			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_33_29856_s_27	15941713	A number of regulatory sites have been identified including a GATA binding site ( ), Sp1 and Sp3 binding sites ( ,  ), as well as a NF-kappaB site ( ) shown to be involved in basal transcriptional activity.	bind
50666	4	11588	6	NULL	NULL	0	NULL		NULL		is involved in	NULL			NF-kappaB site	transcriptional activity	NULL	basal			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_33_29856_s_27	15941713	A number of regulatory sites have been identified including a GATA binding site ( ), Sp1 and Sp3 binding sites ( ,  ), as well as a NF-kappaB site ( ) shown to be involved in basal transcriptional activity.	bind
54219	5	11588	6	10	NULL	0	NULL				is a type of				GATA binding site	regulatory site					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_33_29856_s_27	15941713	A number of regulatory sites have been identified including a GATA binding site ( ), Sp1 and Sp3 binding sites ( ,  ), as well as a NF-kappaB site ( ) shown to be involved in basal transcriptional activity.	bind
54220	6	11588	6	10	NULL	0	NULL				is a type of				Sp1 binding site	regulatory site					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_33_29856_s_27	15941713	A number of regulatory sites have been identified including a GATA binding site ( ), Sp1 and Sp3 binding sites ( ,  ), as well as a NF-kappaB site ( ) shown to be involved in basal transcriptional activity.	bind
54221	7	11588	6	10	NULL	0	NULL				is a type of				Sp3 binding site	regulatory site					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_33_29856_s_27	15941713	A number of regulatory sites have been identified including a GATA binding site ( ), Sp1 and Sp3 binding sites ( ,  ), as well as a NF-kappaB site ( ) shown to be involved in basal transcriptional activity.	bind
54222	8	11588	6	10	NULL	0	NULL				is a type of				NF-kappaB site	regulatory site					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_33_29856_s_27	15941713	A number of regulatory sites have been identified including a GATA binding site ( ), Sp1 and Sp3 binding sites ( ,  ), as well as a NF-kappaB site ( ) shown to be involved in basal transcriptional activity.	bind
51329	1	11589	5	NULL	NULL	NULL	NULL	TAFI	GP		bind			Gly336;;Tyr341;;Glu363		plasminogen	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_8_6620_s_317	14660622	A number of residues in the His333-Val401 region have been reported to be involved in substrate binding (Gly336, Tyr341, and Glu363) ( ), but these three amino acids are conserved in both TAFI and pancreatic pro-CPB, suggesting that residues other than these are important for plasminogen and fibrinogen binding.	bind
51330	2	11589	5	NULL	NULL	NULL	NULL	TAFI	GP		bind			Gly336;;Tyr341;;Glu363		fibrinogen	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_8_6620_s_317	14660622	A number of residues in the His333-Val401 region have been reported to be involved in substrate binding (Gly336, Tyr341, and Glu363) ( ), but these three amino acids are conserved in both TAFI and pancreatic pro-CPB, suggesting that residues other than these are important for plasminogen and fibrinogen binding.	bind
51331	3	11589	5	NULL	NULL	NULL	NULL	pro-CPB	GP	pancreatic	bind			Gly336;;Tyr341;;Glu363		plasminogen	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_8_6620_s_317	14660622	A number of residues in the His333-Val401 region have been reported to be involved in substrate binding (Gly336, Tyr341, and Glu363) ( ), but these three amino acids are conserved in both TAFI and pancreatic pro-CPB, suggesting that residues other than these are important for plasminogen and fibrinogen binding.	bind
51332	4	11589	5	NULL	NULL	NULL	NULL	pro-CPB	GP	pancreatic	bind			Gly336;;Tyr341;;Glu363		fibrinogen	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_8_6620_s_317	14660622	A number of residues in the His333-Val401 region have been reported to be involved in substrate binding (Gly336, Tyr341, and Glu363) ( ), but these three amino acids are conserved in both TAFI and pancreatic pro-CPB, suggesting that residues other than these are important for plasminogen and fibrinogen binding.	bind
51333	5	11589	5	NULL	NULL	NULL	NULL				is conserved in			Gly336;;Tyr341;;Glu363		TAFI	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_8_6620_s_317	14660622	A number of residues in the His333-Val401 region have been reported to be involved in substrate binding (Gly336, Tyr341, and Glu363) ( ), but these three amino acids are conserved in both TAFI and pancreatic pro-CPB, suggesting that residues other than these are important for plasminogen and fibrinogen binding.	bind
51334	6	11589	5	NULL	NULL	NULL	NULL				is conserved in			Gly336;;Tyr341;;Glu363		pro-CPB	GP	pancreatic			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_8_6620_s_317	14660622	A number of residues in the His333-Val401 region have been reported to be involved in substrate binding (Gly336, Tyr341, and Glu363) ( ), but these three amino acids are conserved in both TAFI and pancreatic pro-CPB, suggesting that residues other than these are important for plasminogen and fibrinogen binding.	bind
51335	1	11590	5	NULL	NULL	NULL	NULL	Rho GTPases	GP		bind					GTP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
51336	2	11590	5	NULL	NULL	NULL	NULL	Rho-kinase/ROKalpha/OCK-II	GP		is a type of					Rho effector	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
51337	3	11590	5	NULL	NULL	NULL	NULL	Rho-kinase/ROKalpha/OCK-II	GP		associate with		specifically			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
51338	4	11590	5	NULL	NULL	NULL	NULL	p160ROCK/ROKbeta/ROCK-I	GP		is an isoform of					Rho-kinase	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
51339	5	11590	5	NULL	NULL	NULL	NULL	p160ROCK/ROKbeta/ROCK-I	GP		is a type of					Rho effector	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
51340	6	11590	5	NULL	NULL	NULL	NULL	p160ROCK/ROKbeta/ROCK-I	GP		associate with		specifically			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
51341	7	11590	5	NULL	NULL	NULL	NULL	PKN 1	GP		is					protein kinase N 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
51342	8	11590	5	NULL	NULL	NULL	NULL	PKN 1	GP		is a type of					Rho effector	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
51343	9	11590	5	NULL	NULL	NULL	NULL	PKN 1	GP		associate with		specifically			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
51344	10	11590	5	NULL	NULL	NULL	NULL	rhophilin	GP		associate with		specifically			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
51345	11	11590	5	NULL	NULL	NULL	NULL	rhotekin	GP		associate with		specifically			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
51346	12	11590	5	NULL	NULL	NULL	NULL	citron	GP		associate with		specifically			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
51347	13	11590	5	NULL	NULL	NULL	NULL	citron kinase	GP		associate with		specifically			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
51348	14	11590	5	NULL	NULL	NULL	NULL	mDia	GP		associate with		specifically			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
51349	15	11590	5	NULL	NULL	NULL	NULL	kinectin	GP		associate with		specifically			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
51350	16	11590	5	NULL	NULL	NULL	NULL	rhophilin	GP		is a type of					Rho effector	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
51351	17	11590	5	NULL	NULL	NULL	NULL	rhotekin	GP		is a type of					Rho effector	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
51352	18	11590	5	NULL	NULL	NULL	NULL	citron	GP		is a type of					Rho effector	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
51353	19	11590	5	NULL	NULL	NULL	NULL	citron kinase	GP		is a type of					Rho effector	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
51354	20	11590	5	NULL	NULL	NULL	NULL	mDia	GP		is a type of					Rho effector	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
51355	21	11590	5	NULL	NULL	NULL	NULL	kinectin	GP		is a type of					Rho effector	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
50667	1	11590	6	NULL	NULL	0	NULL	Rho-kinase/ROKalpha/OCK-II	NULL		is a type of	NULL				Rho effector	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
50668	2	11590	6	NULL	NULL	0	NULL	Rho GTPase	NULL		bind	NULL				GTP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
50669	3	11590	6	NULL	NULL	0	NULL	Rho-kinase/ROKalpha/OCK-II	NULL		associates with	NULL	specifically			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
50670	4	11590	6	NULL	NULL	0	NULL	p160ROCK/ROKbeta/ROCK-I	NULL		is a type of	NULL				Rho effector	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
50671	5	11590	6	10	NULL	0	NULL	p160ROCK/ROKbeta/ROCK-I			is an isoform of					Rho-kinase					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
50672	6	11590	6	NULL	NULL	0	NULL	p160ROCK/ROKbeta/ROCK-I	NULL		associates with	NULL	specifically			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
50673	7	11590	6	10	NULL	0	NULL	PKN 1			associates with		specifically			statement 2					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
50674	8	11590	6	10	NULL	0	NULL	PKN 1			is a type of					Rho effector					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
50675	9	11590	6	10	NULL	0	NULL	PKN 1			is					protein kinase N					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
50676	10	11590	6	NULL	NULL	0	NULL	rhophilin	NULL		is a type of	NULL				Rho effector	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
50677	11	11590	6	NULL	NULL	0	NULL	rhophilin	NULL		associates with	NULL	specifically			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
50678	12	11590	6	NULL	NULL	0	NULL	rhotekin	NULL		is a type of	NULL				Rho effector	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
50679	13	11590	6	10	NULL	0	NULL	rhotekin			associates with		specifically			statement 2					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
50680	14	11590	6	10	NULL	0	NULL	citron			associates with		specifically			statement 2					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
50681	15	11590	6	NULL	NULL	0	NULL	citron	NULL		is a type of	NULL				Rho effector	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
50682	16	11590	6	NULL	NULL	0	NULL	citron kinase	NULL		is a type of	NULL				Rho effector	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
50683	17	11590	6	10	NULL	0	NULL	citron kinase			associates with		specifically			statement 2					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
50684	18	11590	6	10	NULL	0	NULL	mDia			associates with		specifically			statement 2					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
50685	19	11590	6	NULL	NULL	0	NULL	mDia	NULL		is a type of	NULL				Rho effector	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
50686	20	11590	6	NULL	NULL	0	NULL	kinectin	NULL		is a type of	NULL				Rho effector	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
50687	21	11590	6	NULL	NULL	0	NULL	kinectin	NULL		associates with	NULL	specifically			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_46046_s_11	12954645	A number of Rho effectors have been identified which associate specifically with the GTP-bound forms of Rho GTPases, including Rho-kinase/ROKalpha/OCK-II, p160ROCK/ROKbeta/ROCK-I (an isoform of Rho-kinase) ( - ), protein kinase N (PKN)  1 ( ,  ), rhophilin ( ), rhotekin ( ), citron ( ), citron kinase ( ), mDia ( ), and kinectin ( ).	bind
51356	1	11591	5	NULL	NULL	NULL	NULL	p56 lck	GP		is involved in					TCR/CD3-dependent signal transduction pathway	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_32_28714_s_9	12045189	A number of signal transducers known to be involved in the TCR/CD3-dependent signal transduction pathway, including p56 lck, p36 lat, and SLP-76, as well as capacitative entry of calcium, are crucial for the noticed CD43 co-stimulatory effect.	bind
51357	2	11591	5	NULL	NULL	NULL	NULL	p36 lat	GP		is involved in					TCR/CD3-dependent signal transduction pathway	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_32_28714_s_9	12045189	A number of signal transducers known to be involved in the TCR/CD3-dependent signal transduction pathway, including p56 lck, p36 lat, and SLP-76, as well as capacitative entry of calcium, are crucial for the noticed CD43 co-stimulatory effect.	bind
51358	3	11591	5	NULL	NULL	NULL	NULL	SLP-76	GP		is involved in					TCR/CD3-dependent signal transduction pathway	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_32_28714_s_9	12045189	A number of signal transducers known to be involved in the TCR/CD3-dependent signal transduction pathway, including p56 lck, p36 lat, and SLP-76, as well as capacitative entry of calcium, are crucial for the noticed CD43 co-stimulatory effect.	bind
51359	4	11591	5	NULL	NULL	NULL	NULL	p56 lck	GP		is a type of					signal transducer	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_32_28714_s_9	12045189	A number of signal transducers known to be involved in the TCR/CD3-dependent signal transduction pathway, including p56 lck, p36 lat, and SLP-76, as well as capacitative entry of calcium, are crucial for the noticed CD43 co-stimulatory effect.	bind
51360	5	11591	5	NULL	NULL	NULL	NULL	p36 lat	GP		is a type of					signal transducer	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_32_28714_s_9	12045189	A number of signal transducers known to be involved in the TCR/CD3-dependent signal transduction pathway, including p56 lck, p36 lat, and SLP-76, as well as capacitative entry of calcium, are crucial for the noticed CD43 co-stimulatory effect.	bind
51361	6	11591	5	NULL	NULL	NULL	NULL	SLP-76	GP		is a type of					signal transducer	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_32_28714_s_9	12045189	A number of signal transducers known to be involved in the TCR/CD3-dependent signal transduction pathway, including p56 lck, p36 lat, and SLP-76, as well as capacitative entry of calcium, are crucial for the noticed CD43 co-stimulatory effect.	bind
50688	1	11591	6	NULL	NULL	0	NULL	p56 lck	NULL		is involved in	NULL				TCR/CD3-dependent signal transduction pathway	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_32_28714_s_9	12045189	A number of signal transducers known to be involved in the TCR/CD3-dependent signal transduction pathway, including p56 lck, p36 lat, and SLP-76, as well as capacitative entry of calcium, are crucial for the noticed CD43 co-stimulatory effect.	bind
50689	2	11591	6	NULL	NULL	0	NULL	p36 lat	NULL		is involved in	NULL				TCR/CD3-dependent signal transduction pathway	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_32_28714_s_9	12045189	A number of signal transducers known to be involved in the TCR/CD3-dependent signal transduction pathway, including p56 lck, p36 lat, and SLP-76, as well as capacitative entry of calcium, are crucial for the noticed CD43 co-stimulatory effect.	bind
50690	3	11591	6	NULL	NULL	0	NULL	SLP-76	NULL		is involved in	NULL				TCR/CD3-dependent signal transduction pathway	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_32_28714_s_9	12045189	A number of signal transducers known to be involved in the TCR/CD3-dependent signal transduction pathway, including p56 lck, p36 lat, and SLP-76, as well as capacitative entry of calcium, are crucial for the noticed CD43 co-stimulatory effect.	bind
54223	4	11591	6	10	NULL	0	NULL	p56 lck			is a type of					signal transducer					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_32_28714_s_9	12045189	A number of signal transducers known to be involved in the TCR/CD3-dependent signal transduction pathway, including p56 lck, p36 lat, and SLP-76, as well as capacitative entry of calcium, are crucial for the noticed CD43 co-stimulatory effect.	bind
54224	5	11591	6	10	NULL	0	NULL	p36 lat			is a type of					signal transducer					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_32_28714_s_9	12045189	A number of signal transducers known to be involved in the TCR/CD3-dependent signal transduction pathway, including p56 lck, p36 lat, and SLP-76, as well as capacitative entry of calcium, are crucial for the noticed CD43 co-stimulatory effect.	bind
54225	6	11591	6	10	NULL	0	NULL	SLP-76			is a type of					signal transducer					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_32_28714_s_9	12045189	A number of signal transducers known to be involved in the TCR/CD3-dependent signal transduction pathway, including p56 lck, p36 lat, and SLP-76, as well as capacitative entry of calcium, are crucial for the noticed CD43 co-stimulatory effect.	bind
51363	1	11593	5	NULL	NULL	NULL	NULL	bFGF	GP		bind					heparin	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17711_s_191	8663454	A number of studies have pointed to the importance of 2- O-sulfated iduronic acid in binding of bFGF to heparin ( 45) and heparan sulfate ( 5,  46).	bind
51364	2	11593	5	NULL	NULL	NULL	NULL	bFGF	GP		bind					heparan sulfate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17711_s_191	8663454	A number of studies have pointed to the importance of 2- O-sulfated iduronic acid in binding of bFGF to heparin ( 45) and heparan sulfate ( 5,  46).	bind
51365	3	11593	5	NULL	NULL	NULL	NULL	2- O-sulfated iduronic acid	Chemical		is important for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17711_s_191	8663454	A number of studies have pointed to the importance of 2- O-sulfated iduronic acid in binding of bFGF to heparin ( 45) and heparan sulfate ( 5,  46).	bind
51366	4	11593	5	NULL	NULL	NULL	NULL	2- O-sulfated iduronic acid	Chemical		is important for					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17711_s_191	8663454	A number of studies have pointed to the importance of 2- O-sulfated iduronic acid in binding of bFGF to heparin ( 45) and heparan sulfate ( 5,  46).	bind
50691	1	11593	6	NULL	NULL	0	NULL	bFGF	NULL		bind	NULL				heparin	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_30_17711_s_191	8663454	A number of studies have pointed to the importance of 2- O-sulfated iduronic acid in binding of bFGF to heparin ( 45) and heparan sulfate ( 5,  46).	bind
50692	2	11593	6	NULL	NULL	0	NULL	bFGF	NULL		bind	NULL				heparan sulfate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_30_17711_s_191	8663454	A number of studies have pointed to the importance of 2- O-sulfated iduronic acid in binding of bFGF to heparin ( 45) and heparan sulfate ( 5,  46).	bind
50693	3	11593	6	NULL	NULL	0	NULL	2- O-sulfated iduronic acid	NULL		plays a role in	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_30_17711_s_191	8663454	A number of studies have pointed to the importance of 2- O-sulfated iduronic acid in binding of bFGF to heparin ( 45) and heparan sulfate ( 5,  46).	bind
50694	4	11593	6	NULL	NULL	0	NULL	2- O-sulfated iduronic acid	NULL		plays a role in	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_30_17711_s_191	8663454	A number of studies have pointed to the importance of 2- O-sulfated iduronic acid in binding of bFGF to heparin ( 45) and heparan sulfate ( 5,  46).	bind
51369	1	11594	5	NULL	NULL	NULL	NULL	CPT I	GP	rat;;liver	contains								malonyl-CoA binding sites		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_11_9058_s_23	12499375	A number of studies have shown that in rat liver CPT I there are two malonyl-CoA binding sites: one with greater capacity for binding and regulation of the inhibitor and not susceptible to competition from acyl-CoA, which behaves as an allosteric component ( 8-12); and a second acyl-CoA binding site, which is located near the catalytic  site ( 13).	bind
50695	1	11594	6	10	NULL	0	NULL	CPT I		rat;; liver	contains								malonyl-CoA binding sites		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_11_9058_s_23	12499375	A number of studies have shown that in rat liver CPT I there are two malonyl-CoA binding sites: one with greater capacity for binding and regulation of the inhibitor and not susceptible to competition from acyl-CoA, which behaves as an allosteric component ( 8-12); and a second acyl-CoA binding site, which is located near the catalytic  site ( 13).	bind
51367	1	11595	5	NULL	NULL	NULL	NULL	NGF	GP		bind					p75	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_61_4_710_s_282	11901208	A number of studies in other cell types have demonstrated the apoptosis-inducing effect of NGF binding to p75 (Kuner and Hertel, 1998  ; Sedel et al., 1999  ).	bind
51368	2	11595	5	NULL	NULL	NULL	NULL	apoptosis	Process		induce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_61_4_710_s_282	11901208	A number of studies in other cell types have demonstrated the apoptosis-inducing effect of NGF binding to p75 (Kuner and Hertel, 1998  ; Sedel et al., 1999  ).	bind
50696	1	11595	6	NULL	NULL	0	NULL	NGF	NULL		bind	NULL				p75	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_4_710_s_282	11901208	A number of studies in other cell types have demonstrated the apoptosis-inducing effect of NGF binding to p75 (Kuner and Hertel, 1998  ; Sedel et al., 1999  ).	bind
50697	2	11595	6	NULL	NULL	0	NULL	apoptosis	NULL		induces	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_4_710_s_282	11901208	A number of studies in other cell types have demonstrated the apoptosis-inducing effect of NGF binding to p75 (Kuner and Hertel, 1998  ; Sedel et al., 1999  ).	bind
51372	1	11596	5	NULL	NULL	NULL	NULL	collagen	GP		bind					GPVI	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
51373	2	11596	5	NULL	NULL	NULL	NULL	CRP	GP		bind					GPVI	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
51374	3	11596	5	NULL	NULL	NULL	NULL	Cvx	GP		bind					GPVI	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
51375	4	11596	5	NULL	NULL	NULL	NULL	statement 1	Process		induce					platelet	Cell	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
51376	5	11596	5	NULL	NULL	NULL	NULL	statement 2	Process		induce					platelet	Cell	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
51377	6	11596	5	NULL	NULL	NULL	NULL	statement 3	Process		induce					platelet	Cell	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
51378	7	11596	5	NULL	NULL	NULL	NULL	statement 4	Process		occurs through					Fc receptor gamma-chain	GP	phosphorylation of	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
51379	8	11596	5	NULL	NULL	NULL	NULL	statement 4	Process		occurs through					Syk	GP	phosphorylation of	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
51380	9	11596	5	NULL	NULL	NULL	NULL	statement 4	Process		occurs through					phospholipase C	GP	phosphorylation of	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
51381	10	11596	5	NULL	NULL	NULL	NULL	statement 5	Process		occurs through					Fc receptor gamma-chain	GP	phosphorylation of	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
51382	11	11596	5	NULL	NULL	NULL	NULL	statement 5	Process		occurs through					Syk	GP	phosphorylation of	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
51383	12	11596	5	NULL	NULL	NULL	NULL	statement 5	Process		occurs through					phospholipase C	GP	phosphorylation of	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
51384	13	11596	5	NULL	NULL	NULL	NULL	statement 6	Process		occurs through					Fc receptor gamma-chain	GP	phosphorylation of	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
51385	14	11596	5	NULL	NULL	NULL	NULL	statement 6	Process		occurs through					Syk	GP	phosphorylation of	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
51386	15	11596	5	NULL	NULL	NULL	NULL	statement 6	Process		occurs through					phospholipase C	GP	phosphorylation of	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
51387	16	11596	5	NULL	NULL	NULL	NULL	collagen	GP		induce					platelet	Cell	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
51388	17	11596	5	NULL	NULL	NULL	NULL	GPVI	GP		is a key receptor for					statement 16	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
50698	1	11596	6	NULL	NULL	0	NULL	collagen	NULL		bind	NULL				GPVI	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
50699	2	11596	6	NULL	NULL	0	NULL	CRP	NULL		bind	NULL				GPVI	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
50700	3	11596	6	NULL	NULL	0	NULL	Cvx	NULL		bind	NULL				GPVI	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
50701	4	11596	6	NULL	NULL	0	NULL	statement 1	NULL		induces	NULL				platelet	NULL	activation of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
50702	5	11596	6	NULL	NULL	0	NULL	statement 2	NULL		induces	NULL				platelet	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
50703	6	11596	6	NULL	NULL	0	NULL	statement 3	NULL		induces	NULL				platelet	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
50704	7	11596	6	NULL	NULL	0	NULL	statement 4	NULL		occurs via	NULL				Fc receptor gamma-chain	NULL	phosphorylation of 	Tyrosine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
50705	8	11596	6	NULL	NULL	0	NULL	statement 4	NULL		occurs via	NULL				Syk	NULL	phosphorylation of	Tyrosine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
50706	9	11596	6	NULL	NULL	0	NULL	statement 4	NULL		occurs via	NULL				phospholipase C	NULL	phosphorylation of	Tyrosine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
50707	10	11596	6	NULL	NULL	0	NULL	statement 5	NULL		occurs via	NULL				Fc receptor gamma-chain	NULL	phosphorylation of	Tyrosine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
50708	11	11596	6	NULL	NULL	0	NULL	statement 5	NULL		occurs via	NULL				Syk	NULL	phosphorylation of	Tyrosine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
50709	12	11596	6	NULL	NULL	0	NULL	statement 5	NULL		occurs via	NULL				phospholipase C	NULL	phosphorylation of	Tyrosine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
50710	13	11596	6	NULL	NULL	0	NULL	statement 6	NULL		occurs via	NULL				Fc receptor gamma-chain	NULL	phosphorylation of	Tyrosine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
50711	14	11596	6	NULL	NULL	0	NULL	statement 6	NULL		occurs via	NULL				Syk	NULL	phosphorylation of	Tyrosine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
50712	15	11596	6	NULL	NULL	0	NULL	statement 6	NULL		occurs via	NULL				phospholipase C	NULL	phosphorylation of	Tyrosine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
50713	16	11596	6	NULL	NULL	0	NULL	collagen	NULL		induces	NULL				platelet	NULL	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
50714	17	11596	6	NULL	NULL	0	NULL	GPVI	NULL		is a key receptor for	NULL				statement 16	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_48_46197_s_21	12356768	A number of studies showed that the binding of collagen, CRP, and Cvx to GPVI induced platelet activation through tyrosine phosphorylation of the Fc receptor gamma-chain, Syk, phospholipase C ,and many other proteins ( 10), thus indicating that GPVI is a key receptor for collagen-induced platelet activation.	bind
51389	1	11597	5	NULL	NULL	NULL	NULL	histone H1	GP		bind		weakly					consensus		NFI-binding sites	NULL		NULL	NULL	NULL	NULL	gw60_gene_249_1_31_s_185	10831836	A number of studies suggest that histone H1 can bind weakly to consensus NFI-binding sites, and that NFI may activate transcription by direct displacement of histone binding at such sites (   Gao and   Ristiniemi).	bind
51390	2	11597	5	NULL	NULL	NULL	NULL	NFI	GP		activate		may			transcription	Process				NULL		NULL	NULL	NULL	NULL	gw60_gene_249_1_31_s_185	10831836	A number of studies suggest that histone H1 can bind weakly to consensus NFI-binding sites, and that NFI may activate transcription by direct displacement of histone binding at such sites (   Gao and   Ristiniemi).	bind
51392	3	11597	5	NULL	NULL	NULL	NULL	NFI	GP		displaces		directly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_gene_249_1_31_s_185	10831836	A number of studies suggest that histone H1 can bind weakly to consensus NFI-binding sites, and that NFI may activate transcription by direct displacement of histone binding at such sites (   Gao and   Ristiniemi).	bind
51393	4	11597	5	NULL	NULL	NULL	NULL	statement 3	Process		leads to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_gene_249_1_31_s_185	10831836	A number of studies suggest that histone H1 can bind weakly to consensus NFI-binding sites, and that NFI may activate transcription by direct displacement of histone binding at such sites (   Gao and   Ristiniemi).	bind
50715	1	11597	6	NULL	NULL	0	NULL	histone H1	NULL		bind	NULL	weakly				NULL	consensus		NFI-binding sites	NULL		0	NULL	NULL	NULL	gw60_gene_249_1_31_s_185	10831836	A number of studies suggest that histone H1 can bind weakly to consensus NFI-binding sites, and that NFI may activate transcription by direct displacement of histone binding at such sites (   Gao and   Ristiniemi).	bind
50716	2	11597	6	NULL	NULL	0	NULL	NFI	NULL		displace	NULL	directly			histone H1	NULL				NULL	statement 1	NULL	NULL	NULL	NULL	gw60_gene_249_1_31_s_185	10831836	A number of studies suggest that histone H1 can bind weakly to consensus NFI-binding sites, and that NFI may activate transcription by direct displacement of histone binding at such sites (   Gao and   Ristiniemi).	bind
50717	3	11597	6	NULL	NULL	0	NULL	NFI	NULL		activate	NULL	may			transcription	NULL				NULL		0	NULL	NULL	NULL	gw60_gene_249_1_31_s_185	10831836	A number of studies suggest that histone H1 can bind weakly to consensus NFI-binding sites, and that NFI may activate transcription by direct displacement of histone binding at such sites (   Gao and   Ristiniemi).	bind
50718	4	11597	6	NULL	NULL	0	NULL	statement 3	NULL		occurs via	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_gene_249_1_31_s_185	10831836	A number of studies suggest that histone H1 can bind weakly to consensus NFI-binding sites, and that NFI may activate transcription by direct displacement of histone binding at such sites (   Gao and   Ristiniemi).	bind
51420	1	11598	5	NULL	NULL	NULL	NULL	TRX2 gene	GP		encodes					thioredoxin	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_7_1710_s_26	9130715	A number of such targets have now been identified, including the  TRX2 gene which encodes thioredoxin that confers increased resistance to oxidative stress (Kuge and Jones, 1994  ),  YCF1 which encodes an ATP-binding cassette transporter gene essential for cadmium tolerance (Wemmie  et al., 1994a  ),  GSH1 which encodes gamma-glutamylcysteine synthetase involved in glutathione biosynthesis (Wu and Moye-Rowley, 1994  ),  GLR1 which encodes glutathione reductase (Grant  et al., 1996  ), and the additional ABC transporter proteins  PDR5 and  SNQ2 (Miyahara  et al., 1996  ).	bind
51421	2	11598	5	NULL	NULL	NULL	NULL	TRX2 gene	GP		confers					oxidative stress	Process	increased resistance to			NULL		NULL	NULL	NULL	NULL	gw60_embo_16_7_1710_s_26	9130715	A number of such targets have now been identified, including the  TRX2 gene which encodes thioredoxin that confers increased resistance to oxidative stress (Kuge and Jones, 1994  ),  YCF1 which encodes an ATP-binding cassette transporter gene essential for cadmium tolerance (Wemmie  et al., 1994a  ),  GSH1 which encodes gamma-glutamylcysteine synthetase involved in glutathione biosynthesis (Wu and Moye-Rowley, 1994  ),  GLR1 which encodes glutathione reductase (Grant  et al., 1996  ), and the additional ABC transporter proteins  PDR5 and  SNQ2 (Miyahara  et al., 1996  ).	bind
51422	3	11598	5	NULL	NULL	NULL	NULL	YCF1	GP		encodes					ATP-binding cassette transporter gene	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_7_1710_s_26	9130715	A number of such targets have now been identified, including the  TRX2 gene which encodes thioredoxin that confers increased resistance to oxidative stress (Kuge and Jones, 1994  ),  YCF1 which encodes an ATP-binding cassette transporter gene essential for cadmium tolerance (Wemmie  et al., 1994a  ),  GSH1 which encodes gamma-glutamylcysteine synthetase involved in glutathione biosynthesis (Wu and Moye-Rowley, 1994  ),  GLR1 which encodes glutathione reductase (Grant  et al., 1996  ), and the additional ABC transporter proteins  PDR5 and  SNQ2 (Miyahara  et al., 1996  ).	bind
51423	4	11598	5	NULL	NULL	NULL	NULL	YCF1	GP		is essential for					cadmium 	Chemical	tolerance of			NULL		NULL	NULL	NULL	NULL	gw60_embo_16_7_1710_s_26	9130715	A number of such targets have now been identified, including the  TRX2 gene which encodes thioredoxin that confers increased resistance to oxidative stress (Kuge and Jones, 1994  ),  YCF1 which encodes an ATP-binding cassette transporter gene essential for cadmium tolerance (Wemmie  et al., 1994a  ),  GSH1 which encodes gamma-glutamylcysteine synthetase involved in glutathione biosynthesis (Wu and Moye-Rowley, 1994  ),  GLR1 which encodes glutathione reductase (Grant  et al., 1996  ), and the additional ABC transporter proteins  PDR5 and  SNQ2 (Miyahara  et al., 1996  ).	bind
51424	5	11598	5	NULL	NULL	NULL	NULL	GSH1	GP		encodes					gamma-glutamylcysteine synthetase	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_7_1710_s_26	9130715	A number of such targets have now been identified, including the  TRX2 gene which encodes thioredoxin that confers increased resistance to oxidative stress (Kuge and Jones, 1994  ),  YCF1 which encodes an ATP-binding cassette transporter gene essential for cadmium tolerance (Wemmie  et al., 1994a  ),  GSH1 which encodes gamma-glutamylcysteine synthetase involved in glutathione biosynthesis (Wu and Moye-Rowley, 1994  ),  GLR1 which encodes glutathione reductase (Grant  et al., 1996  ), and the additional ABC transporter proteins  PDR5 and  SNQ2 (Miyahara  et al., 1996  ).	bind
51425	6	11598	5	NULL	NULL	NULL	NULL	gamma-glutamylcysteine synthetase	GP		is involved in					glutathione	Chemical	biosynthesis of			NULL		NULL	NULL	NULL	NULL	gw60_embo_16_7_1710_s_26	9130715	A number of such targets have now been identified, including the  TRX2 gene which encodes thioredoxin that confers increased resistance to oxidative stress (Kuge and Jones, 1994  ),  YCF1 which encodes an ATP-binding cassette transporter gene essential for cadmium tolerance (Wemmie  et al., 1994a  ),  GSH1 which encodes gamma-glutamylcysteine synthetase involved in glutathione biosynthesis (Wu and Moye-Rowley, 1994  ),  GLR1 which encodes glutathione reductase (Grant  et al., 1996  ), and the additional ABC transporter proteins  PDR5 and  SNQ2 (Miyahara  et al., 1996  ).	bind
51426	7	11598	5	NULL	NULL	NULL	NULL	GLR1	GP		encodes					glutathione reductase	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_7_1710_s_26	9130715	A number of such targets have now been identified, including the  TRX2 gene which encodes thioredoxin that confers increased resistance to oxidative stress (Kuge and Jones, 1994  ),  YCF1 which encodes an ATP-binding cassette transporter gene essential for cadmium tolerance (Wemmie  et al., 1994a  ),  GSH1 which encodes gamma-glutamylcysteine synthetase involved in glutathione biosynthesis (Wu and Moye-Rowley, 1994  ),  GLR1 which encodes glutathione reductase (Grant  et al., 1996  ), and the additional ABC transporter proteins  PDR5 and  SNQ2 (Miyahara  et al., 1996  ).	bind
51427	8	11598	5	NULL	NULL	NULL	NULL	PDR5	GP		is a type of					ABC transporter protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_7_1710_s_26	9130715	A number of such targets have now been identified, including the  TRX2 gene which encodes thioredoxin that confers increased resistance to oxidative stress (Kuge and Jones, 1994  ),  YCF1 which encodes an ATP-binding cassette transporter gene essential for cadmium tolerance (Wemmie  et al., 1994a  ),  GSH1 which encodes gamma-glutamylcysteine synthetase involved in glutathione biosynthesis (Wu and Moye-Rowley, 1994  ),  GLR1 which encodes glutathione reductase (Grant  et al., 1996  ), and the additional ABC transporter proteins  PDR5 and  SNQ2 (Miyahara  et al., 1996  ).	bind
51428	9	11598	5	NULL	NULL	NULL	NULL	SNQ2 	GP		is a type of					ABC transporter protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_16_7_1710_s_26	9130715	A number of such targets have now been identified, including the  TRX2 gene which encodes thioredoxin that confers increased resistance to oxidative stress (Kuge and Jones, 1994  ),  YCF1 which encodes an ATP-binding cassette transporter gene essential for cadmium tolerance (Wemmie  et al., 1994a  ),  GSH1 which encodes gamma-glutamylcysteine synthetase involved in glutathione biosynthesis (Wu and Moye-Rowley, 1994  ),  GLR1 which encodes glutathione reductase (Grant  et al., 1996  ), and the additional ABC transporter proteins  PDR5 and  SNQ2 (Miyahara  et al., 1996  ).	bind
50719	1	11598	6	NULL	NULL	0	NULL	TRX2 gene	NULL		encodes	NULL				thioredoxin	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_16_7_1710_s_26	9130715	A number of such targets have now been identified, including the  TRX2 gene which encodes thioredoxin that confers increased resistance to oxidative stress (Kuge and Jones, 1994  ),  YCF1 which encodes an ATP-binding cassette transporter gene essential for cadmium tolerance (Wemmie  et al., 1994a  ),  GSH1 which encodes gamma-glutamylcysteine synthetase involved in glutathione biosynthesis (Wu and Moye-Rowley, 1994  ),  GLR1 which encodes glutathione reductase (Grant  et al., 1996  ), and the additional ABC transporter proteins  PDR5 and  SNQ2 (Miyahara  et al., 1996  ).	bind
50720	2	11598	6	10	NULL	0	NULL	TRX2 gene			confers					oxidative stress		increased resistance to			NULL		NULL	NULL	NULL	NULL	gw60_embo_16_7_1710_s_26	9130715	A number of such targets have now been identified, including the  TRX2 gene which encodes thioredoxin that confers increased resistance to oxidative stress (Kuge and Jones, 1994  ),  YCF1 which encodes an ATP-binding cassette transporter gene essential for cadmium tolerance (Wemmie  et al., 1994a  ),  GSH1 which encodes gamma-glutamylcysteine synthetase involved in glutathione biosynthesis (Wu and Moye-Rowley, 1994  ),  GLR1 which encodes glutathione reductase (Grant  et al., 1996  ), and the additional ABC transporter proteins  PDR5 and  SNQ2 (Miyahara  et al., 1996  ).	bind
50721	3	11598	6	NULL	NULL	0	NULL	YCF1	NULL		encodes	NULL				ATP-binding cassette transporter gene	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_16_7_1710_s_26	9130715	A number of such targets have now been identified, including the  TRX2 gene which encodes thioredoxin that confers increased resistance to oxidative stress (Kuge and Jones, 1994  ),  YCF1 which encodes an ATP-binding cassette transporter gene essential for cadmium tolerance (Wemmie  et al., 1994a  ),  GSH1 which encodes gamma-glutamylcysteine synthetase involved in glutathione biosynthesis (Wu and Moye-Rowley, 1994  ),  GLR1 which encodes glutathione reductase (Grant  et al., 1996  ), and the additional ABC transporter proteins  PDR5 and  SNQ2 (Miyahara  et al., 1996  ).	bind
50722	4	11598	6	10	NULL	0	NULL	statement 3			is essential for					cadmium		 tolerance of			NULL		NULL	NULL	NULL	NULL	gw60_embo_16_7_1710_s_26	9130715	A number of such targets have now been identified, including the  TRX2 gene which encodes thioredoxin that confers increased resistance to oxidative stress (Kuge and Jones, 1994  ),  YCF1 which encodes an ATP-binding cassette transporter gene essential for cadmium tolerance (Wemmie  et al., 1994a  ),  GSH1 which encodes gamma-glutamylcysteine synthetase involved in glutathione biosynthesis (Wu and Moye-Rowley, 1994  ),  GLR1 which encodes glutathione reductase (Grant  et al., 1996  ), and the additional ABC transporter proteins  PDR5 and  SNQ2 (Miyahara  et al., 1996  ).	bind
50723	5	11598	6	NULL	NULL	0	NULL	GSH1	NULL		encodes	NULL				gamma-glutamylcysteine synthetase	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_16_7_1710_s_26	9130715	A number of such targets have now been identified, including the  TRX2 gene which encodes thioredoxin that confers increased resistance to oxidative stress (Kuge and Jones, 1994  ),  YCF1 which encodes an ATP-binding cassette transporter gene essential for cadmium tolerance (Wemmie  et al., 1994a  ),  GSH1 which encodes gamma-glutamylcysteine synthetase involved in glutathione biosynthesis (Wu and Moye-Rowley, 1994  ),  GLR1 which encodes glutathione reductase (Grant  et al., 1996  ), and the additional ABC transporter proteins  PDR5 and  SNQ2 (Miyahara  et al., 1996  ).	bind
50724	6	11598	6	10	NULL	0	NULL	GSH1			is involved in					glutathione 		biosynthesis of			NULL		NULL	NULL	NULL	NULL	gw60_embo_16_7_1710_s_26	9130715	A number of such targets have now been identified, including the  TRX2 gene which encodes thioredoxin that confers increased resistance to oxidative stress (Kuge and Jones, 1994  ),  YCF1 which encodes an ATP-binding cassette transporter gene essential for cadmium tolerance (Wemmie  et al., 1994a  ),  GSH1 which encodes gamma-glutamylcysteine synthetase involved in glutathione biosynthesis (Wu and Moye-Rowley, 1994  ),  GLR1 which encodes glutathione reductase (Grant  et al., 1996  ), and the additional ABC transporter proteins  PDR5 and  SNQ2 (Miyahara  et al., 1996  ).	bind
50725	7	11598	6	NULL	NULL	0	NULL	GLR1	NULL		encodes	NULL				glutathione reductase	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_16_7_1710_s_26	9130715	A number of such targets have now been identified, including the  TRX2 gene which encodes thioredoxin that confers increased resistance to oxidative stress (Kuge and Jones, 1994  ),  YCF1 which encodes an ATP-binding cassette transporter gene essential for cadmium tolerance (Wemmie  et al., 1994a  ),  GSH1 which encodes gamma-glutamylcysteine synthetase involved in glutathione biosynthesis (Wu and Moye-Rowley, 1994  ),  GLR1 which encodes glutathione reductase (Grant  et al., 1996  ), and the additional ABC transporter proteins  PDR5 and  SNQ2 (Miyahara  et al., 1996  ).	bind
54226	8	11598	6	10	NULL	0	NULL	PDR5 			is a type of					ABC transporter protein					NULL		0	NULL	NULL	NULL	gw60_embo_16_7_1710_s_26	9130715	A number of such targets have now been identified, including the  TRX2 gene which encodes thioredoxin that confers increased resistance to oxidative stress (Kuge and Jones, 1994  ),  YCF1 which encodes an ATP-binding cassette transporter gene essential for cadmium tolerance (Wemmie  et al., 1994a  ),  GSH1 which encodes gamma-glutamylcysteine synthetase involved in glutathione biosynthesis (Wu and Moye-Rowley, 1994  ),  GLR1 which encodes glutathione reductase (Grant  et al., 1996  ), and the additional ABC transporter proteins  PDR5 and  SNQ2 (Miyahara  et al., 1996  ).	bind
54227	9	11598	6	10	NULL	0	NULL	SNQ2 			is a type of					ABC transporter protein					NULL		0	NULL	NULL	NULL	gw60_embo_16_7_1710_s_26	9130715	A number of such targets have now been identified, including the  TRX2 gene which encodes thioredoxin that confers increased resistance to oxidative stress (Kuge and Jones, 1994  ),  YCF1 which encodes an ATP-binding cassette transporter gene essential for cadmium tolerance (Wemmie  et al., 1994a  ),  GSH1 which encodes gamma-glutamylcysteine synthetase involved in glutathione biosynthesis (Wu and Moye-Rowley, 1994  ),  GLR1 which encodes glutathione reductase (Grant  et al., 1996  ), and the additional ABC transporter proteins  PDR5 and  SNQ2 (Miyahara  et al., 1996  ).	bind
51394	1	11599	5	NULL	NULL	NULL	NULL	PAI-1 promoter	NucleicAcid		is a type of					TGF-beta/SMAD-regulated promoters	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
51395	2	11599	5	NULL	NULL	NULL	NULL	collagenase I promoter	NucleicAcid		is a type of					TGF-beta/SMAD-regulated promoters	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
51396	3	11599	5	NULL	NULL	NULL	NULL	c-Jun promoter	NucleicAcid		is a type of					TGF-beta/SMAD-regulated promoters	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
51397	4	11599	5	NULL	NULL	NULL	NULL	IgA promoter	NucleicAcid		is a type of					TGF-beta/SMAD-regulated promoters	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
51398	5	11599	5	NULL	NULL	NULL	NULL	Jun B promoter	NucleicAcid		is a type of					TGF-beta/SMAD-regulated promoters	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
51399	6	11599	5	NULL	NULL	NULL	NULL	PAI-1	GP		contains				promoter					GTCT	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
51400	7	11599	5	NULL	NULL	NULL	NULL	PAI-1	GP		contains				promoter					AGAC	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
51401	8	11599	5	NULL	NULL	NULL	NULL	collagenase I	GP		contains				promoter					GTCT	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
51402	9	11599	5	NULL	NULL	NULL	NULL	collagenase I	GP		contains				promoter					AGAC	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
51403	10	11599	5	NULL	NULL	NULL	NULL	c-Jun	GP		contains				promoter					GTCT	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
51404	11	11599	5	NULL	NULL	NULL	NULL	c-Jun	GP		contains				promoter					AGAC	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
51405	12	11599	5	NULL	NULL	NULL	NULL	IgA	GP		contains				promoter					GTCT	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
51406	13	11599	5	NULL	NULL	NULL	NULL	IgA	GP		contains				promoter					AGAC	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
51407	14	11599	5	NULL	NULL	NULL	NULL	Jun B	GP		contains				promoter					AGAC	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
51408	15	11599	5	NULL	NULL	NULL	NULL	Smad3-Smad4 complex	GP		bind					statement 6	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
51409	16	11599	5	NULL	NULL	NULL	NULL	Smad3-Smad4 complex	GP		bind					statement 7	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
51410	17	11599	5	NULL	NULL	NULL	NULL	Smad3-Smad4 complex	GP		bind					statement 8	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
51411	18	11599	5	NULL	NULL	NULL	NULL	Smad3-Smad4 complex	GP		bind					statement 9	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
51412	19	11599	5	NULL	NULL	NULL	NULL	Smad3-Smad4 complex	GP		bind					statement 10	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
51413	20	11599	5	NULL	NULL	NULL	NULL	Smad3-Smad4 complex	GP		bind					statement 11	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
51414	21	11599	5	NULL	NULL	NULL	NULL	Smad3-Smad4 complex	GP		bind					statement 12	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
51415	22	11599	5	NULL	NULL	NULL	NULL	Smad3-Smad4 complex	GP		bind					statement 13	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
51416	23	11599	5	NULL	NULL	NULL	NULL	Smad3-Smad4 complex	GP		bind					statement 14	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
54228	24	11599	5	NULL	NULL	NULL	NULL	Jun B	GP		contains				promoter					GTCT	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
54229	25	11599	5	NULL	NULL	NULL	NULL	Smad3-Smad4 complex	GP		bind					statement 24	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
50726	1	11599	6	NULL	NULL	0	NULL	PAI-1	NULL		contains	NULL			promoter		NULL			GTCT	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
50727	2	11599	6	NULL	NULL	0	NULL	PAI-1	NULL		contains	NULL			promoter		NULL			AGAC	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
50728	3	11599	6	NULL	NULL	0	NULL	collagenase I	NULL		contains	NULL			promoter		NULL			GTCT	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
50729	4	11599	6	NULL	NULL	0	NULL	collagenase I	NULL		contains	NULL			promoter		NULL			AGAC	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
50730	5	11599	6	NULL	NULL	0	NULL	c-Jun	NULL		contains	NULL			promoter		NULL			GTCT	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
50731	6	11599	6	NULL	NULL	0	NULL	c-Jun	NULL		contains	NULL			promoter		NULL			AGAC	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
50732	7	11599	6	NULL	NULL	0	NULL	IgA	NULL		contains	NULL			promoter		NULL			GTCT 	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
50736	8	11599	6	NULL	NULL	0	NULL	IgA	NULL		contains	NULL			promoter		NULL			AGAC	NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
50737	9	11599	6	NULL	NULL	0	NULL	Jun B	NULL		contains	NULL			promoter		NULL			GTCT	NULL		0	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
50738	10	11599	6	NULL	NULL	0	NULL	Jun B	NULL		contains	NULL			promoter		NULL			AGAC	NULL		0	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
50739	11	11599	6	NULL	NULL	0	NULL	Smad3-Smad4 complex	NULL		bind	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
50740	12	11599	6	NULL	NULL	0	NULL	Smad3-Smad4 complex	NULL		bind	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
50741	13	11599	6	NULL	NULL	0	NULL	Smad3-Smad4 complex	NULL		bind	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
50742	14	11599	6	NULL	NULL	0	NULL	Smad3-Smad4 complex	NULL		bind	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
50743	15	11599	6	NULL	NULL	0	NULL	Smad3-Smad4 complex	NULL		bind	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
50744	16	11599	6	NULL	NULL	0	NULL	Smad3-Smad4 complex	NULL		bind	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
50745	17	11599	6	NULL	NULL	0	NULL	Smad3-Smad4 complex	NULL		bind	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
50746	18	11599	6	NULL	NULL	0	NULL	Smad3-Smad4 complex	NULL		bind	NULL				statement 8	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
50747	19	11599	6	NULL	NULL	0	NULL	Smad3-Smad4 complex	NULL		bind	NULL				statement 9	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
50748	20	11599	6	NULL	NULL	0	NULL	Smad3-Smad4 complex	NULL		bind	NULL				statement 10	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
54230	21	11599	6	10	NULL	0	NULL	PAI-1			is a type of					TGF-beta/SMAD-regulated promoter					NULL		0	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
54231	22	11599	6	10	NULL	0	NULL	collagenase I			is a type of					TGF-beta/SMAD-regulated promoter					NULL		0	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
54232	23	11599	6	10	NULL	0	NULL	c-Jun			is a type of					TGF-beta/SMAD-regulated promoter					NULL		0	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
54234	24	11599	6	10	NULL	0	NULL	IgA			is a type of					TGF-beta/SMAD-regulated promoter					NULL		0	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
54235	25	11599	6	10	NULL	0	NULL	Jun B			is a type of					TGF-beta/SMAD-regulated promoter					NULL		0	NULL	NULL	NULL	gw60_pnas_97_12_6397_s_17	10823886	A number of TGF-beta/SMAD-regulated promoters, such as the PAI-1, collagenase I, c-Jun, IgA, and Jun B promoters, contain one or multiple copies of the sequence GTCT or AGAC, which can be bound by the Smad3-Smad4 complex ( 15-24).	bind
51417	1	11600	5	NULL	NULL	NULL	NULL	SOS	GP		bind			proline-rich sequences		Grb2	GP		SH3 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_32_30552_s_283	11375989	A number of these are linked to intracellular signaling complexes found near the plasma membrane, for example, proline-rich sequences of SOS bind to the SH3 domains of Grb2, and this leads to the activation of ras and is therefore required for growth factor signaling ( 37).	bind
51418	2	11600	5	NULL	NULL	NULL	NULL	statement 1	Process		activates					ras	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_32_30552_s_283	11375989	A number of these are linked to intracellular signaling complexes found near the plasma membrane, for example, proline-rich sequences of SOS bind to the SH3 domains of Grb2, and this leads to the activation of ras and is therefore required for growth factor signaling ( 37).	bind
51419	3	11600	5	NULL	NULL	NULL	NULL	statement 1	Process		is required for					growth factor	GP	signaling of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_32_30552_s_283	11375989	A number of these are linked to intracellular signaling complexes found near the plasma membrane, for example, proline-rich sequences of SOS bind to the SH3 domains of Grb2, and this leads to the activation of ras and is therefore required for growth factor signaling ( 37).	bind
50733	1	11600	6	NULL	NULL	0	NULL	SOS	NULL		bind	NULL		proline rich sequences		Grb2	NULL		SH3 domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_32_30552_s_283	11375989	A number of these are linked to intracellular signaling complexes found near the plasma membrane, for example, proline-rich sequences of SOS bind to the SH3 domains of Grb2, and this leads to the activation of ras and is therefore required for growth factor signaling ( 37).	bind
50734	2	11600	6	10	NULL	0	NULL	statement 1			activates					ras					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_32_30552_s_283	11375989	A number of these are linked to intracellular signaling complexes found near the plasma membrane, for example, proline-rich sequences of SOS bind to the SH3 domains of Grb2, and this leads to the activation of ras and is therefore required for growth factor signaling ( 37).	bind
50735	3	11600	6	10	NULL	0	NULL	statement 2			is required for					growth factor 		signaling of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_32_30552_s_283	11375989	A number of these are linked to intracellular signaling complexes found near the plasma membrane, for example, proline-rich sequences of SOS bind to the SH3 domains of Grb2, and this leads to the activation of ras and is therefore required for growth factor signaling ( 37).	bind
67985	1	333026	5	NULL	NULL	NULL	NULL	CCZ1	GP		is a synonym of					YBR131w	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_biochem-biophys-res-commun_329_1_15721293_s_2	15721293	The CCZ1 (YBR131w) gene encodes a protein required for fusion of various  transport intermediates with the vacuole.	gene_phenotype
67986	2	333026	5	NULL	NULL	0	NULL	transport intermediates	AbstractConcept		fuse with					vacuole	CellComponent				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_biochem-biophys-res-commun_329_1_15721293_s_2	15721293	The CCZ1 (YBR131w) gene encodes a protein required for fusion of various  transport intermediates with the vacuole.	gene_phenotype
67987	1	333027	5	NULL	NULL	0	NULL	SEC4 gene	GP		encodes					Rab proteins	GP				NULL	yeast	0	NULL	NULL	NULL	gw60_jbiolchem_273_6_3253_s_15	9452439	Eleven genes encoding Rab proteins ( SEC4,  YPT1,  YPT31,  YPT32,  YPT51,  YPT52,  YPT53,  YPT6,  YPT7,  YBR264C, and  YNL304W) are found in yeast where they play important roles in vesicle transport.	gene_phenotype
67988	2	333027	5	NULL	NULL	NULL	NULL	SEC4 gene	GP		plays a role in		important			vesicle	CellComponent	transport of			NULL	yeast	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_6_3253_s_15	9452439	Eleven genes encoding Rab proteins ( SEC4,  YPT1,  YPT31,  YPT32,  YPT51,  YPT52,  YPT53,  YPT6,  YPT7,  YBR264C, and  YNL304W) are found in yeast where they play important roles in vesicle transport.	gene_phenotype
67989	3	333027	5	NULL	NULL	0	NULL	YPT1 gene	GP		encodes					Rab proteins	GP				NULL	yeast	0	NULL	NULL	NULL	gw60_jbiolchem_273_6_3253_s_15	9452439	Eleven genes encoding Rab proteins ( SEC4,  YPT1,  YPT31,  YPT32,  YPT51,  YPT52,  YPT53,  YPT6,  YPT7,  YBR264C, and  YNL304W) are found in yeast where they play important roles in vesicle transport.	gene_phenotype
67990	4	333027	5	NULL	NULL	NULL	NULL	YPT1 gene	GP		plays a role in		important			vesicle	CellComponent	transport of			NULL	yeast	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_6_3253_s_15	9452439	Eleven genes encoding Rab proteins ( SEC4,  YPT1,  YPT31,  YPT32,  YPT51,  YPT52,  YPT53,  YPT6,  YPT7,  YBR264C, and  YNL304W) are found in yeast where they play important roles in vesicle transport.	gene_phenotype
67991	5	333027	5	NULL	NULL	0	NULL	YPT31 gene	GP		encodes					Rab proteins	GP				NULL	yeast	0	NULL	NULL	NULL	gw60_jbiolchem_273_6_3253_s_15	9452439	Eleven genes encoding Rab proteins ( SEC4,  YPT1,  YPT31,  YPT32,  YPT51,  YPT52,  YPT53,  YPT6,  YPT7,  YBR264C, and  YNL304W) are found in yeast where they play important roles in vesicle transport.	gene_phenotype
67992	6	333027	5	NULL	NULL	0	NULL	YPT31 gene	GP		plays a role in		important			vesicle	CellComponent	transport of			NULL	yeast	0	NULL	NULL	NULL	gw60_jbiolchem_273_6_3253_s_15	9452439	Eleven genes encoding Rab proteins ( SEC4,  YPT1,  YPT31,  YPT32,  YPT51,  YPT52,  YPT53,  YPT6,  YPT7,  YBR264C, and  YNL304W) are found in yeast where they play important roles in vesicle transport.	gene_phenotype
67993	7	333027	5	NULL	NULL	0	NULL	YPT32 gene	GP		encodes					Rab proteins	GP				NULL	yeast	0	NULL	NULL	NULL	gw60_jbiolchem_273_6_3253_s_15	9452439	Eleven genes encoding Rab proteins ( SEC4,  YPT1,  YPT31,  YPT32,  YPT51,  YPT52,  YPT53,  YPT6,  YPT7,  YBR264C, and  YNL304W) are found in yeast where they play important roles in vesicle transport.	gene_phenotype
67994	8	333027	5	NULL	NULL	0	NULL	YPT32 gene	GP		plays a role in		important			vesicle	CellComponent	transport of			NULL	yeast	0	NULL	NULL	NULL	gw60_jbiolchem_273_6_3253_s_15	9452439	Eleven genes encoding Rab proteins ( SEC4,  YPT1,  YPT31,  YPT32,  YPT51,  YPT52,  YPT53,  YPT6,  YPT7,  YBR264C, and  YNL304W) are found in yeast where they play important roles in vesicle transport.	gene_phenotype
67995	9	333027	5	NULL	NULL	0	NULL	YPT51 gene	GP		encodes					Rab proteins	GP				NULL	yeast	0	NULL	NULL	NULL	gw60_jbiolchem_273_6_3253_s_15	9452439	Eleven genes encoding Rab proteins ( SEC4,  YPT1,  YPT31,  YPT32,  YPT51,  YPT52,  YPT53,  YPT6,  YPT7,  YBR264C, and  YNL304W) are found in yeast where they play important roles in vesicle transport.	gene_phenotype
67996	10	333027	5	NULL	NULL	0	NULL	YPT51 gene	GP		plays a role in		important			vesicle	GP	transport of			NULL	yeast	0	NULL	NULL	NULL	gw60_jbiolchem_273_6_3253_s_15	9452439	Eleven genes encoding Rab proteins ( SEC4,  YPT1,  YPT31,  YPT32,  YPT51,  YPT52,  YPT53,  YPT6,  YPT7,  YBR264C, and  YNL304W) are found in yeast where they play important roles in vesicle transport.	gene_phenotype
67997	11	333027	5	NULL	NULL	0	NULL	YPT52 gene	GP		encodes					Rab proteins	GP				NULL	yeast	0	NULL	NULL	NULL	gw60_jbiolchem_273_6_3253_s_15	9452439	Eleven genes encoding Rab proteins ( SEC4,  YPT1,  YPT31,  YPT32,  YPT51,  YPT52,  YPT53,  YPT6,  YPT7,  YBR264C, and  YNL304W) are found in yeast where they play important roles in vesicle transport.	gene_phenotype
67998	12	333027	5	NULL	NULL	0	NULL	YPT52 gene	GP		plays a role in		important			vesicle	CellComponent	transport of			NULL	yeast	0	NULL	NULL	NULL	gw60_jbiolchem_273_6_3253_s_15	9452439	Eleven genes encoding Rab proteins ( SEC4,  YPT1,  YPT31,  YPT32,  YPT51,  YPT52,  YPT53,  YPT6,  YPT7,  YBR264C, and  YNL304W) are found in yeast where they play important roles in vesicle transport.	gene_phenotype
67999	13	333027	5	NULL	NULL	0	NULL	YPT53 gene	GP		encodes					Rab proteins	GP				NULL	yeast	0	NULL	NULL	NULL	gw60_jbiolchem_273_6_3253_s_15	9452439	Eleven genes encoding Rab proteins ( SEC4,  YPT1,  YPT31,  YPT32,  YPT51,  YPT52,  YPT53,  YPT6,  YPT7,  YBR264C, and  YNL304W) are found in yeast where they play important roles in vesicle transport.	gene_phenotype
68000	14	333027	5	NULL	NULL	0	NULL	YPT53 gene	GP		plays a role in		important			vesicle	CellComponent	transport of			NULL	yeast	0	NULL	NULL	NULL	gw60_jbiolchem_273_6_3253_s_15	9452439	Eleven genes encoding Rab proteins ( SEC4,  YPT1,  YPT31,  YPT32,  YPT51,  YPT52,  YPT53,  YPT6,  YPT7,  YBR264C, and  YNL304W) are found in yeast where they play important roles in vesicle transport.	gene_phenotype
68001	15	333027	5	NULL	NULL	0	NULL	YPT6 gene	GP		encodes					Rab proteins	GP				NULL	yeast	0	NULL	NULL	NULL	gw60_jbiolchem_273_6_3253_s_15	9452439	Eleven genes encoding Rab proteins ( SEC4,  YPT1,  YPT31,  YPT32,  YPT51,  YPT52,  YPT53,  YPT6,  YPT7,  YBR264C, and  YNL304W) are found in yeast where they play important roles in vesicle transport.	gene_phenotype
68002	16	333027	5	NULL	NULL	0	NULL	YPT6 gene	GP		plays a role in		important			vesicle	CellComponent	transport of			NULL	yeast	0	NULL	NULL	NULL	gw60_jbiolchem_273_6_3253_s_15	9452439	Eleven genes encoding Rab proteins ( SEC4,  YPT1,  YPT31,  YPT32,  YPT51,  YPT52,  YPT53,  YPT6,  YPT7,  YBR264C, and  YNL304W) are found in yeast where they play important roles in vesicle transport.	gene_phenotype
68003	17	333027	5	NULL	NULL	0	NULL	YPT7 gene	GP		encodes					Rab proteins	GP				NULL	yeast	0	NULL	NULL	NULL	gw60_jbiolchem_273_6_3253_s_15	9452439	Eleven genes encoding Rab proteins ( SEC4,  YPT1,  YPT31,  YPT32,  YPT51,  YPT52,  YPT53,  YPT6,  YPT7,  YBR264C, and  YNL304W) are found in yeast where they play important roles in vesicle transport.	gene_phenotype
68004	18	333027	5	NULL	NULL	0	NULL	YPT7 gene	GP		plays a role in		important			vesicle	CellComponent	transport of			NULL	yeast	0	NULL	NULL	NULL	gw60_jbiolchem_273_6_3253_s_15	9452439	Eleven genes encoding Rab proteins ( SEC4,  YPT1,  YPT31,  YPT32,  YPT51,  YPT52,  YPT53,  YPT6,  YPT7,  YBR264C, and  YNL304W) are found in yeast where they play important roles in vesicle transport.	gene_phenotype
68005	19	333027	5	NULL	NULL	0	NULL	YBR264C gene	GP		encodes					Rab proteins	GP				NULL	yeast	0	NULL	NULL	NULL	gw60_jbiolchem_273_6_3253_s_15	9452439	Eleven genes encoding Rab proteins ( SEC4,  YPT1,  YPT31,  YPT32,  YPT51,  YPT52,  YPT53,  YPT6,  YPT7,  YBR264C, and  YNL304W) are found in yeast where they play important roles in vesicle transport.	gene_phenotype
68006	20	333027	5	NULL	NULL	0	NULL	YBR264C gene	GP		plays a role in		important			vesicle	CellComponent	transport of			NULL	yeast	0	NULL	NULL	NULL	gw60_jbiolchem_273_6_3253_s_15	9452439	Eleven genes encoding Rab proteins ( SEC4,  YPT1,  YPT31,  YPT32,  YPT51,  YPT52,  YPT53,  YPT6,  YPT7,  YBR264C, and  YNL304W) are found in yeast where they play important roles in vesicle transport.	gene_phenotype
68007	21	333027	5	NULL	NULL	0	NULL	YNL304W gene	GP		encodes					Rab proteins	GP				NULL	yeast	0	NULL	NULL	NULL	gw60_jbiolchem_273_6_3253_s_15	9452439	Eleven genes encoding Rab proteins ( SEC4,  YPT1,  YPT31,  YPT32,  YPT51,  YPT52,  YPT53,  YPT6,  YPT7,  YBR264C, and  YNL304W) are found in yeast where they play important roles in vesicle transport.	gene_phenotype
68008	22	333027	5	NULL	NULL	0	NULL	YNL304W gene	GP		plays a role in		important			vesicle	CellComponent	transport of			NULL	yeast	0	NULL	NULL	NULL	gw60_jbiolchem_273_6_3253_s_15	9452439	Eleven genes encoding Rab proteins ( SEC4,  YPT1,  YPT31,  YPT32,  YPT51,  YPT52,  YPT53,  YPT6,  YPT7,  YBR264C, and  YNL304W) are found in yeast where they play important roles in vesicle transport.	gene_phenotype
68009	1	333030	5	NULL	NULL	0	NULL	YDR330W	AminoAcid		is homologous to					ubiquitin regulatory protein domains	AminoAcid				NULL		0	NULL	NULL	NULL	gw60_pnas_97_1_262_s_222	10618406	In the proteasome class, YDR330W has homology to ubiquitin regulatory protein domains, suggesting a role in ubiquitin-dependent proteasome activity.	gene_phenotype
68010	2	333030	5	NULL	NULL	0	NULL	proteasome	GP	activity of	is dependent on					ubiquitin	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_97_1_262_s_222	10618406	In the proteasome class, YDR330W has homology to ubiquitin regulatory protein domains, suggesting a role in ubiquitin-dependent proteasome activity.	gene_phenotype
68011	3	333030	5	NULL	NULL	0	NULL	statement 1	Process		plays a role in		may			statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_97_1_262_s_222	10618406	In the proteasome class, YDR330W has homology to ubiquitin regulatory protein domains, suggesting a role in ubiquitin-dependent proteasome activity.	gene_phenotype
68012	1	333031	5	NULL	NULL	0	NULL	Csm1	GP		interacts with		might			Lrs4 protein	GP				NULL		0	NULL	NULL	NULL	gw60_devcell_4_4_535_s_88	12689592	Genome-wide two-hybrid data  (Uetz et al., 2000  ) raised the possibility that Csm1 might interact with a protein called Lrs4 (loss of rDNA silencing; product of ORF YDR439W) that had been implicated in rDNA silencing  (Smith et al., 1999  ).	gene_phenotype
68013	2	333031	5	NULL	NULL	0	NULL	Lrs4	GP		is					loss of rDNA silencing	GP				NULL		0	NULL	NULL	NULL	gw60_devcell_4_4_535_s_88	12689592	Genome-wide two-hybrid data  (Uetz et al., 2000  ) raised the possibility that Csm1 might interact with a protein called Lrs4 (loss of rDNA silencing; product of ORF YDR439W) that had been implicated in rDNA silencing  (Smith et al., 1999  ).	gene_phenotype
68014	3	333031	5	NULL	NULL	0	NULL	Lrs4 protein	GP		is a product of					ORF	NucleicAcid		YDR439W		NULL		0	NULL	NULL	NULL	gw60_devcell_4_4_535_s_88	12689592	Genome-wide two-hybrid data  (Uetz et al., 2000  ) raised the possibility that Csm1 might interact with a protein called Lrs4 (loss of rDNA silencing; product of ORF YDR439W) that had been implicated in rDNA silencing  (Smith et al., 1999  ).	gene_phenotype
68015	4	333031	5	NULL	NULL	0	NULL	Lrs4 protein	GP		is implicated in					rDNA	NucleicAcid	silencing of			NULL		0	NULL	NULL	NULL	gw60_devcell_4_4_535_s_88	12689592	Genome-wide two-hybrid data  (Uetz et al., 2000  ) raised the possibility that Csm1 might interact with a protein called Lrs4 (loss of rDNA silencing; product of ORF YDR439W) that had been implicated in rDNA silencing  (Smith et al., 1999  ).	gene_phenotype
68016	1	333033	5	NULL	NULL	NULL	NULL	MAD2 gene	GP	budding yeast S. cerevisiae	is a type of					spindle checkpoint gene	GP	budding yeast S. cerevisiae			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_8_2607_s_79	10436016	The spindle checkpoint gene  MAD2 in the budding yeast  S. cerevisiae was originally identified (Li and Murray, 1991  ) as the ORF YJL031C, which encodes a subunit of an essential prenyltransferase (Li  et al., 1993  ) and has been renamed  BET4.	gene_phenotype
68017	2	333033	5	NULL	NULL	0	NULL	MAD2 gene	GP	budding yeast S. cerevisiae	is					ORF	NucleicAcid		YJL031C		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_10_8_2607_s_79	10436016	The spindle checkpoint gene  MAD2 in the budding yeast  S. cerevisiae was originally identified (Li and Murray, 1991  ) as the ORF YJL031C, which encodes a subunit of an essential prenyltransferase (Li  et al., 1993  ) and has been renamed  BET4.	gene_phenotype
68018	3	333033	5	NULL	NULL	0	NULL	MAD2 gene	GP	budding yeast S. cerevisiae	encodes					prenyltransferase	GP	subunit of;;essential			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_10_8_2607_s_79	10436016	The spindle checkpoint gene  MAD2 in the budding yeast  S. cerevisiae was originally identified (Li and Murray, 1991  ) as the ORF YJL031C, which encodes a subunit of an essential prenyltransferase (Li  et al., 1993  ) and has been renamed  BET4.	gene_phenotype
68019	4	333033	5	NULL	NULL	NULL	NULL	MAD2 gene	GP	budding yeast S. cerevisiae	is renamed as					BET4	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_10_8_2607_s_79	10436016	The spindle checkpoint gene  MAD2 in the budding yeast  S. cerevisiae was originally identified (Li and Murray, 1991  ) as the ORF YJL031C, which encodes a subunit of an essential prenyltransferase (Li  et al., 1993  ) and has been renamed  BET4.	gene_phenotype
68020	1	333034	5	NULL	NULL	0	NULL	Cnb1	GP		is a subunit of		regulatory	YKL190W		calcineurin	GP	S. cerevisiae			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_13_12231_s_79	15657058	A BLAST program search using the peptide sequence of Cnb1 (YKL190W), the regulatory subunit of calcineurin of  S. cerevisiae ( ,  ), against the  S. pombe protein data base at the Sanger Center revealed an open reading frame, SPCC830.06, which except for the N- and C-terminal domains, exhibits a significant similarity to the budding yeast Cnb1 (score = 680,  p = 8.7e - 69, identities = 142/174 (81%)).	gene_phenotype
68022	2	333034	5	NULL	NULL	0	NULL	Cnb1	GP	S. cerevisiae	is similar to		significantly			SPCC830.06	NucleicAcid	S. pombe			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_13_12231_s_79	15657058	A BLAST program search using the peptide sequence of Cnb1 (YKL190W), the regulatory subunit of calcineurin of  S. cerevisiae ( ,  ), against the  S. pombe protein data base at the Sanger Center revealed an open reading frame, SPCC830.06, which except for the N- and C-terminal domains, exhibits a significant similarity to the budding yeast Cnb1 (score = 680,  p = 8.7e - 69, identities = 142/174 (81%)).	gene_phenotype
68023	3	333034	5	NULL	NULL	0	NULL	SPCC830.06	NucleicAcid		is a type of					open reading frame	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_13_12231_s_79	15657058	A BLAST program search using the peptide sequence of Cnb1 (YKL190W), the regulatory subunit of calcineurin of  S. cerevisiae ( ,  ), against the  S. pombe protein data base at the Sanger Center revealed an open reading frame, SPCC830.06, which except for the N- and C-terminal domains, exhibits a significant similarity to the budding yeast Cnb1 (score = 680,  p = 8.7e - 69, identities = 142/174 (81%)).	gene_phenotype
68024	1	333036	5	NULL	NULL	0	NULL	CTR2	GP		encodes				orf19.4720	copper transporter	GP	putative			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4814_s_229	16030247	We also see prolonged induction of  CTR2 (orf19.4720), which encodes a putative copper transporter;  YOL075C (orf19.3120), which encodes a putative ferric cation transporter; and  YMR209C (orf19.4816), which encodes a protein of unknown function that contains a GMP kinase domain.	gene_phenotype
68028	2	333036	5	NULL	NULL	0	NULL				encodes			YOL075C	orf19.3120	ferric cation transporter	GP	putative			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4814_s_229	16030247	We also see prolonged induction of  CTR2 (orf19.4720), which encodes a putative copper transporter;  YOL075C (orf19.3120), which encodes a putative ferric cation transporter; and  YMR209C (orf19.4816), which encodes a protein of unknown function that contains a GMP kinase domain.	gene_phenotype
68029	3	333036	5	NULL	NULL	0	NULL				encodes			YMR209C	orf19.4816	protein	GP		GMP kinase domain		NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_10_4814_s_229	16030247	We also see prolonged induction of  CTR2 (orf19.4720), which encodes a putative copper transporter;  YOL075C (orf19.3120), which encodes a putative ferric cation transporter; and  YMR209C (orf19.4816), which encodes a protein of unknown function that contains a GMP kinase domain.	gene_phenotype
68030	1	333037	5	NULL	NULL	0	NULL	Abp140p	GP		is not homologous to					actin binding protein	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_99_2_751_s_27	11805329	Abp140p does not show homology to any known actin binding protein and is expressed in cells by fusion of two ORFs (YOR239W and YOR240W) by means of a +1 translational frameshift.	gene_phenotype
68031	2	333037	5	NULL	NULL	0	NULL	ORF	NucleicAcid		is fused to			YOR239W		ORF	NucleicAcid		YOR240W		NULL		0	NULL	NULL	NULL	gw60_pnas_99_2_751_s_27	11805329	Abp140p does not show homology to any known actin binding protein and is expressed in cells by fusion of two ORFs (YOR239W and YOR240W) by means of a +1 translational frameshift.	gene_phenotype
68032	3	333037	5	NULL	NULL	0	NULL	statement 2	Process		leads to					Abp140p	GP	expression of			NULL	cells	0	NULL	NULL	NULL	gw60_pnas_99_2_751_s_27	11805329	Abp140p does not show homology to any known actin binding protein and is expressed in cells by fusion of two ORFs (YOR239W and YOR240W) by means of a +1 translational frameshift.	gene_phenotype
68033	4	333037	5	NULL	NULL	0	NULL	+1 translational frameshift	Process		leads to					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_99_2_751_s_27	11805329	Abp140p does not show homology to any known actin binding protein and is expressed in cells by fusion of two ORFs (YOR239W and YOR240W) by means of a +1 translational frameshift.	gene_phenotype
68034	1	333038	5	NULL	NULL	NULL	NULL	sterol transport	Process	subcellular	is conserved in					yeast cells	Cell				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_164_4_547_s_41	14970192	Subcellular sterol transport may also be conserved between yeast and mammalian cells; Ncr1p (YPL006w) is an uncharacterized 1,170-residue transmembrane protein with a signal peptide, eight N-glycosylation sites, and 35% identity to the human Npc1 protein.	gene_phenotype
68035	2	333038	5	NULL	NULL	0	NULL	sterol transport	Process	subcellular	is conserved in					mammalian cells	Cell				NULL		0	NULL	NULL	NULL	gw70_cellbiol_164_4_547_s_41	14970192	Subcellular sterol transport may also be conserved between yeast and mammalian cells; Ncr1p (YPL006w) is an uncharacterized 1,170-residue transmembrane protein with a signal peptide, eight N-glycosylation sites, and 35% identity to the human Npc1 protein.	gene_phenotype
68036	3	333038	5	NULL	NULL	0	NULL	Ncr1p	GP		is a type of			YPL006w		1,170-residue transmembrane protein	GP	uncharacterized			NULL		0	NULL	NULL	NULL	gw70_cellbiol_164_4_547_s_41	14970192	Subcellular sterol transport may also be conserved between yeast and mammalian cells; Ncr1p (YPL006w) is an uncharacterized 1,170-residue transmembrane protein with a signal peptide, eight N-glycosylation sites, and 35% identity to the human Npc1 protein.	gene_phenotype
68037	4	333038	5	NULL	NULL	0	NULL	Ncr1p	GP		consists of			YPL006w					signal peptide;;N-glycosylation sites		NULL		0	NULL	NULL	NULL	gw70_cellbiol_164_4_547_s_41	14970192	Subcellular sterol transport may also be conserved between yeast and mammalian cells; Ncr1p (YPL006w) is an uncharacterized 1,170-residue transmembrane protein with a signal peptide, eight N-glycosylation sites, and 35% identity to the human Npc1 protein.	gene_phenotype
68038	5	333038	5	NULL	NULL	0	NULL	Ncr1p	GP		is similar to			YPL006w		Npc1 protein	GP	human			NULL		0	NULL	NULL	NULL	gw70_cellbiol_164_4_547_s_41	14970192	Subcellular sterol transport may also be conserved between yeast and mammalian cells; Ncr1p (YPL006w) is an uncharacterized 1,170-residue transmembrane protein with a signal peptide, eight N-glycosylation sites, and 35% identity to the human Npc1 protein.	gene_phenotype
68039	1	333040	5	NULL	NULL	0	NULL	YPR007C	AminoAcid		is a part of					sporulation cluster	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_18_0_829_s_223	10837077	Indeed, the essential  role in sporulation for one of the previously uncharacterized genes in the sporulation  cluster, YPR007C, which is predicted to encode a putative chromosome cohesion protein,  was established following its identification by this cluster analysis method ( 40).	gene_phenotype
68040	2	333040	5	NULL	NULL	0	NULL	YPR007C	AminoAcid		encodes		potentially			chromosome cohesion protein	GP	putative			NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_18_0_829_s_223	10837077	Indeed, the essential  role in sporulation for one of the previously uncharacterized genes in the sporulation  cluster, YPR007C, which is predicted to encode a putative chromosome cohesion protein,  was established following its identification by this cluster analysis method ( 40).	gene_phenotype
68091	1	333042	5	NULL	NULL	0	NULL	Bcp1	GP		is a homolog of					BCCIP	GP	S. cerevisiae			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_5_1949_s_283	15713648	The  S. cerevisiae BCCIP homolog, Bcp1 (open reading frame number YDR361C), is essential for viability ( ) (Saccharomyces Genome Database at  http://www.yeastgenome.	gene_phenotype
68092	2	333042	5	NULL	NULL	0	NULL	Bcp1	GP		is essential for			YDR361C		viability	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_5_1949_s_283	15713648	The  S. cerevisiae BCCIP homolog, Bcp1 (open reading frame number YDR361C), is essential for viability ( ) (Saccharomyces Genome Database at  http://www.yeastgenome.	gene_phenotype
68093	1	333043	5	NULL	NULL	0	NULL	YDR374C	AminoAcid		is required for					sporulation	Process	efficient			NULL		0	NULL	NULL	NULL	gw60_pnas_99_21_13431_s_133	12370439	Indeed, two of these ( YDR374C and  SLZ1) have recently been shown in genome-wide deletion analysis to be required for efficient sporulation (A. Deutschbauer and R.W.D., unpublished data).	gene_phenotype
68094	2	333043	5	NULL	NULL	0	NULL	SLZ1	GP		is required for					sporulation	Process	efficient			NULL		0	NULL	NULL	NULL	gw60_pnas_99_21_13431_s_133	12370439	Indeed, two of these ( YDR374C and  SLZ1) have recently been shown in genome-wide deletion analysis to be required for efficient sporulation (A. Deutschbauer and R.W.D., unpublished data).	gene_phenotype
68095	1	333044	5	NULL	NULL	NULL	NULL	MAM1	GP		is					monopolar microtubule attachment during meiosis I	GP				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_7_1155_s_45	11163190	This paper concentrates on the role of just one  of these, a gene called  MAM1 ( monopolar microtubule  attachment during  meiosis I, ORF: YER106W), whose deletion  has no effect on vegetative growth but has extraordinary consequences during meiosis.	gene_phenotype
68096	2	333044	5	NULL	NULL	0	NULL	MAM1 gene	GP	deletion of	does not effect			YER106W	ORF	vegetative growth	Process				NULL		0	NULL	NULL	NULL	gw60_cell_103_7_1155_s_45	11163190	This paper concentrates on the role of just one  of these, a gene called  MAM1 ( monopolar microtubule  attachment during  meiosis I, ORF: YER106W), whose deletion  has no effect on vegetative growth but has extraordinary consequences during meiosis.	gene_phenotype
68097	3	333044	5	NULL	NULL	NULL	NULL	MAM1 gene	GP	deletion of	effects		extraordinary	YER106W	ORF	meiosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_103_7_1155_s_45	11163190	This paper concentrates on the role of just one  of these, a gene called  MAM1 ( monopolar microtubule  attachment during  meiosis I, ORF: YER106W), whose deletion  has no effect on vegetative growth but has extraordinary consequences during meiosis.	gene_phenotype
68098	1	333045	5	NULL	NULL	0	NULL	MAM1	GP		is necessary for			YER106W		sister kinetochores	Chromosome	monopolar attachment of			NULL		0	NULL	NULL	NULL	gw60_currbiol_11_13_1001_s_141	11470404	One of these ( YER106W, which we called  MAM1) has been analyzed in detail and been shown to be necessary for monopolar attachment of sister kinetochores during meiosis I  [4  .	gene_phenotype
68099	2	333045	5	NULL	NULL	0	NULL	statement 1	Process		occurs during					meiosis	Process				NULL		0	NULL	NULL	NULL	gw60_currbiol_11_13_1001_s_141	11470404	One of these ( YER106W, which we called  MAM1) has been analyzed in detail and been shown to be necessary for monopolar attachment of sister kinetochores during meiosis I  [4  .	gene_phenotype
68100	1	333046	5	NULL	NULL	0	NULL	HOP2 gene	GP	upregulated	is involved in					meiosis	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68101	2	333046	5	NULL	NULL	0	NULL	HOP2 gene	GP	upregulated	is involved in					sporulation	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68102	3	333046	5	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68103	4	333046	5	NULL	NULL	0	NULL	IME2 gene	GP	upregulated	is involved in					meiosis	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68104	5	333046	5	NULL	NULL	0	NULL	IME2 gene	GP	upregulated	is involved in					sporulation	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68105	6	333046	5	NULL	NULL	0	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68106	7	333046	5	NULL	NULL	0	NULL	REC102 gene	GP	upregulated	is involved in					meiosis	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68107	8	333046	5	NULL	NULL	0	NULL	REC102 gene	GP	upregulated	is involved in					sporulation	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68108	9	333046	5	NULL	NULL	0	NULL	statement 7	Process		is an alternative to					statement 8	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68109	10	333046	5	NULL	NULL	0	NULL	REC104 gene	GP	upregulated	is involved in					meiosis	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68110	11	333046	5	NULL	NULL	0	NULL	REC104 gene	GP	upregulated	is involved in					sporulation	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68111	12	333046	5	NULL	NULL	0	NULL	statement 10	Process		is an alternative to					statement 11	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68112	13	333046	5	NULL	NULL	0	NULL	RED1 gene	GP	upregulated	is involved in					meiosis	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68113	14	333046	5	NULL	NULL	0	NULL	RED1 gene	GP	upregulated	is involved in					sporulation	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68114	15	333046	5	NULL	NULL	0	NULL	statement 13	Process		is an alternative to					statement 12	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68115	16	333046	5	NULL	NULL	0	NULL	SLZ1 gene	GP	upregulated	is involved in					meiosis	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68116	17	333046	5	NULL	NULL	0	NULL	SLZ1 gene	GP	upregulated	is involved in					sporulation	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68117	18	333046	5	NULL	NULL	0	NULL	statement 16	Process		is an alternative to					statement 17	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68118	19	333046	5	NULL	NULL	0	NULL	SPO13 gene	GP	upregulated	is involved in					meiosis	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68119	20	333046	5	NULL	NULL	0	NULL	SPO13 gene	GP	upregulated	is involved in					sporulation	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68120	21	333046	5	NULL	NULL	0	NULL	statement 19	Process		is an alternative to					statement 20	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68121	22	333046	5	NULL	NULL	0	NULL	SPO16 gene	GP	upregulated	is involved in					meiosis	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68122	23	333046	5	NULL	NULL	0	NULL	SPO16 gene	GP	upregulated	is involved in					sporulation	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68123	24	333046	5	NULL	NULL	0	NULL	statement 22	Process		is an alternative to					statement 23	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68124	25	333046	5	NULL	NULL	0	NULL	SPR1 gene	GP	upregulated	is involved in					meiosis	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68125	26	333046	5	NULL	NULL	0	NULL	SPR1 gene	GP	upregulated	is involved in					sporulation	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68126	27	333046	5	NULL	NULL	0	NULL	statement 25	Process		is an alternative to					statement 26	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68127	28	333046	5	NULL	NULL	0	NULL	YER179W	AminoAcid	upregulated	is involved in					meiosis	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68128	29	333046	5	NULL	NULL	0	NULL	YER179W	AminoAcid	upregulated	is involved in					sporulation	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68129	30	333046	5	NULL	NULL	0	NULL	statement 28	Process		is an alternative to					statement 29	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68130	31	333046	5	NULL	NULL	0	NULL	ZIP1 gene	GP	upregulated	is involved in					meiosis	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68131	32	333046	5	NULL	NULL	0	NULL	ZIP1 gene	GP	upregulated	is involved in					sporulation	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68132	33	333046	5	NULL	NULL	0	NULL	statement 31	Process		is an alternative to					statement 32	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_1_159_s_112	14711638	These upregulated genes included 11 that were involved in meiosis or sporulation ( HOP2,  IME2,  REC102,  REC104,  RED1,  SLZ1,  SPO13,  SPO16,  SPR1,  YER179W, and  ZIP1).	gene_phenotype
68133	1	333048	5	NULL	NULL	0	NULL	YNL124W	AminoAcid		is involved in					RNA processing	Process				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_301_3_633_s_87	12565826	In  a similar example, we suggest that YNL124W and YIL104C are involved in RNA processing  and modification ( Fig. 4B).	gene_phenotype
68134	2	333048	5	NULL	NULL	0	NULL	YNL124W	AminoAcid		is involved in					RNA modification	Process				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_301_3_633_s_87	12565826	In  a similar example, we suggest that YNL124W and YIL104C are involved in RNA processing  and modification ( Fig. 4B).	gene_phenotype
68135	3	333048	5	NULL	NULL	0	NULL	YIL104C	AminoAcid		is involved in					RNA processing	Process				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_301_3_633_s_87	12565826	In  a similar example, we suggest that YNL124W and YIL104C are involved in RNA processing  and modification ( Fig. 4B).	gene_phenotype
68136	4	333048	5	NULL	NULL	0	NULL	YIL104C	AminoAcid		is involved in					RNA modification	Process				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_301_3_633_s_87	12565826	In  a similar example, we suggest that YNL124W and YIL104C are involved in RNA processing  and modification ( Fig. 4B).	gene_phenotype
68137	1	333049	5	NULL	NULL	NULL	NULL	taurocholate	Chemical		is translocated across					vacuolar membranes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_febslett_520_1_63_s_20	12044871	The Ybt1p/Bat1p ( YLL048c) transporter translocates taurocholate and other bile acids across vacuolar membranes [  29].	gene_phenotype
68138	2	333049	5	NULL	NULL	0	NULL	bile acids	Chemical		is translocated across					vacuolar membranes	CellComponent				NULL		0	NULL	NULL	NULL	gw60_febslett_520_1_63_s_20	12044871	The Ybt1p/Bat1p ( YLL048c) transporter translocates taurocholate and other bile acids across vacuolar membranes [  29].	gene_phenotype
68139	3	333049	5	NULL	NULL	0	NULL	Ybt1p/Bat1p transporter	GP		is required for			YLL048c		statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_520_1_63_s_20	12044871	The Ybt1p/Bat1p ( YLL048c) transporter translocates taurocholate and other bile acids across vacuolar membranes [  29].	gene_phenotype
68140	4	333049	5	NULL	NULL	0	NULL	Ybt1p/Bat1p transporter	GP		is required for			YLL048c		statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_520_1_63_s_20	12044871	The Ybt1p/Bat1p ( YLL048c) transporter translocates taurocholate and other bile acids across vacuolar membranes [  29].	gene_phenotype
68141	1	333050	5	NULL	NULL	NULL	NULL	PCH2	GP	splicing efficiency of	is similar to			YBR186W				splicing efficiency of	YDL115C		NULL	vegetative diploids	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_8_1700_s_205	10734188	Five other new introns in meiotic genes we have tested (YBR186W/ PCH2, YDL115C, YLR093C/ NYV1 YLR211C and YNL012W/ SPO1; see Table  1) all appear to have similar splicing efficiencies in vegetative and sporulating diploids (data not shown), suggesting that their splicing is not selectively activated during meiosis.	gene_phenotype
68142	2	333050	5	NULL	NULL	0	NULL	PCH2	GP	splicing efficiency of	is similar to			YBR186W				splicing efficiency of	YDL115C		NULL	sporulating diploids	0	NULL	NULL	NULL	gw60_nucleicacidsres_28_8_1700_s_205	10734188	Five other new introns in meiotic genes we have tested (YBR186W/ PCH2, YDL115C, YLR093C/ NYV1 YLR211C and YNL012W/ SPO1; see Table  1) all appear to have similar splicing efficiencies in vegetative and sporulating diploids (data not shown), suggesting that their splicing is not selectively activated during meiosis.	gene_phenotype
68143	3	333050	5	NULL	NULL	0	NULL	NYV1	GP	splicing efficiency of	is similar to			YLR093C				splicing efficiency of	YLR211C		NULL	vegetative diploids	0	NULL	NULL	NULL	gw60_nucleicacidsres_28_8_1700_s_205	10734188	Five other new introns in meiotic genes we have tested (YBR186W/ PCH2, YDL115C, YLR093C/ NYV1 YLR211C and YNL012W/ SPO1; see Table  1) all appear to have similar splicing efficiencies in vegetative and sporulating diploids (data not shown), suggesting that their splicing is not selectively activated during meiosis.	gene_phenotype
68144	4	333050	5	NULL	NULL	NULL	NULL	NYV1	GP	splicing efficiency of	is similar to			YLR093C				splicing efficiency of	YLR211C		NULL	sporulating diploids	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_8_1700_s_205	10734188	Five other new introns in meiotic genes we have tested (YBR186W/ PCH2, YDL115C, YLR093C/ NYV1 YLR211C and YNL012W/ SPO1; see Table  1) all appear to have similar splicing efficiencies in vegetative and sporulating diploids (data not shown), suggesting that their splicing is not selectively activated during meiosis.	gene_phenotype
68145	5	333050	5	NULL	NULL	0	NULL	PCH2	GP	splicing efficiency of	is similar to			YBR186W		NYV1	GP	splicing efficiency of	YLR093C		NULL	vegetative diploids	0	NULL	NULL	NULL	gw60_nucleicacidsres_28_8_1700_s_205	10734188	Five other new introns in meiotic genes we have tested (YBR186W/ PCH2, YDL115C, YLR093C/ NYV1 YLR211C and YNL012W/ SPO1; see Table  1) all appear to have similar splicing efficiencies in vegetative and sporulating diploids (data not shown), suggesting that their splicing is not selectively activated during meiosis.	gene_phenotype
68146	6	333050	5	NULL	NULL	0	NULL	PCH2	GP	splicing efficiency of	is similar to			YBR186W		NYV1	GP	splicing efficiency of	YLR093C		NULL	sporulating diploids	0	NULL	NULL	NULL	gw60_nucleicacidsres_28_8_1700_s_205	10734188	Five other new introns in meiotic genes we have tested (YBR186W/ PCH2, YDL115C, YLR093C/ NYV1 YLR211C and YNL012W/ SPO1; see Table  1) all appear to have similar splicing efficiencies in vegetative and sporulating diploids (data not shown), suggesting that their splicing is not selectively activated during meiosis.	gene_phenotype
68147	7	333050	5	NULL	NULL	NULL	NULL	PCH2	GP	splicing efficiency of	is similar to			YBR186W		SPO1	GP	splicing efficiency of	YNL012W		NULL	vegetative diploids	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_8_1700_s_205	10734188	Five other new introns in meiotic genes we have tested (YBR186W/ PCH2, YDL115C, YLR093C/ NYV1 YLR211C and YNL012W/ SPO1; see Table  1) all appear to have similar splicing efficiencies in vegetative and sporulating diploids (data not shown), suggesting that their splicing is not selectively activated during meiosis.	gene_phenotype
68148	8	333050	5	NULL	NULL	NULL	NULL	PCH2	GP	splicing efficiency of	is similar to			YBR186W		SPO1	GP	splicing efficiency of	YNL012W		NULL	sporulating diploids	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_8_1700_s_205	10734188	Five other new introns in meiotic genes we have tested (YBR186W/ PCH2, YDL115C, YLR093C/ NYV1 YLR211C and YNL012W/ SPO1; see Table  1) all appear to have similar splicing efficiencies in vegetative and sporulating diploids (data not shown), suggesting that their splicing is not selectively activated during meiosis.	gene_phenotype
68250	1	333051	5	NULL	NULL	0	NULL	YLR127c	NucleicAcid		is a type of					ORF	NucleicAcid				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_yeast_16_15_11054824_s_4	11054824	Two ORFs, YLR127c and YLR129w, are essential for viability,  whereas no growth phenotype could be detected following deletion of YLR124w,  YLR125w, YLR126c or YLR128w.	gene_phenotype
68251	2	333051	5	NULL	NULL	0	NULL	YLR129w	NucleicAcid		is a type of					ORF	NucleicAcid				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_yeast_16_15_11054824_s_4	11054824	Two ORFs, YLR127c and YLR129w, are essential for viability,  whereas no growth phenotype could be detected following deletion of YLR124w,  YLR125w, YLR126c or YLR128w.	gene_phenotype
68252	3	333051	5	NULL	NULL	0	NULL	YLR127c	NucleicAcid		is essential for					viability	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_yeast_16_15_11054824_s_4	11054824	Two ORFs, YLR127c and YLR129w, are essential for viability,  whereas no growth phenotype could be detected following deletion of YLR124w,  YLR125w, YLR126c or YLR128w.	gene_phenotype
68253	4	333051	5	NULL	NULL	0	NULL	YLR129w	NucleicAcid		is essential for					viability	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_yeast_16_15_11054824_s_4	11054824	Two ORFs, YLR127c and YLR129w, are essential for viability,  whereas no growth phenotype could be detected following deletion of YLR124w,  YLR125w, YLR126c or YLR128w.	gene_phenotype
68254	5	333051	5	NULL	NULL	0	NULL	YLR124w	NucleicAcid	deletion of	leads to					growth phenotype		absence of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_yeast_16_15_11054824_s_4	11054824	Two ORFs, YLR127c and YLR129w, are essential for viability,  whereas no growth phenotype could be detected following deletion of YLR124w,  YLR125w, YLR126c or YLR128w.	gene_phenotype
68255	6	333051	5	NULL	NULL	0	NULL	YLR125w	NucleicAcid	deletion of	leads to					growth phenotype		absence of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_yeast_16_15_11054824_s_4	11054824	Two ORFs, YLR127c and YLR129w, are essential for viability,  whereas no growth phenotype could be detected following deletion of YLR124w,  YLR125w, YLR126c or YLR128w.	gene_phenotype
68256	7	333051	5	NULL	NULL	0	NULL	YLR126c	NucleicAcid	deletion of	leads to					growth phenotype		absence of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_yeast_16_15_11054824_s_4	11054824	Two ORFs, YLR127c and YLR129w, are essential for viability,  whereas no growth phenotype could be detected following deletion of YLR124w,  YLR125w, YLR126c or YLR128w.	gene_phenotype
68257	8	333051	5	NULL	NULL	0	NULL	YLR128w	NucleicAcid	deletion of	leads to					growth phenotype		absence of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_yeast_16_15_11054824_s_4	11054824	Two ORFs, YLR127c and YLR129w, are essential for viability,  whereas no growth phenotype could be detected following deletion of YLR124w,  YLR125w, YLR126c or YLR128w.	gene_phenotype
68258	1	333053	5	NULL	NULL	0	NULL	YMR101c	NucleicAcid		is a type of					open reading frame	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_1_471_s_204	9858571	This DNA fragment contained a single open reading frame (YMR101c) encoding a protein of 343 amino acids and was able to complement the temperature-sensitive growth of the  rer2 mutant on a single-copy plasmid.	gene_phenotype
68259	2	333053	5	NULL	NULL	0	NULL	YMR101c	NucleicAcid		encodes					protein of 343 amino acids	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_1_471_s_204	9858571	This DNA fragment contained a single open reading frame (YMR101c) encoding a protein of 343 amino acids and was able to complement the temperature-sensitive growth of the  rer2 mutant on a single-copy plasmid.	gene_phenotype
68260	3	333053	5	NULL	NULL	NULL	NULL	rer2	GP	mutant;;growth of	is sensitive to					temperature					NULL	single-copy plasmid	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_471_s_204	9858571	This DNA fragment contained a single open reading frame (YMR101c) encoding a protein of 343 amino acids and was able to complement the temperature-sensitive growth of the  rer2 mutant on a single-copy plasmid.	gene_phenotype
68261	4	333053	5	NULL	NULL	0	NULL	YMR101c	NucleicAcid		complements					statement 3	Process				NULL	single-copy plasmid	0	NULL	NULL	NULL	gw60_molcellbiol_19_1_471_s_204	9858571	This DNA fragment contained a single open reading frame (YMR101c) encoding a protein of 343 amino acids and was able to complement the temperature-sensitive growth of the  rer2 mutant on a single-copy plasmid.	gene_phenotype
68262	1	333054	5	NULL	NULL	0	NULL	ADE17	GP		encodes					isozyme of 5-aminoimidazole-4-carboxamide ribonucleotide transformylase	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_97_22_12369_s_114	11035792	The remaining four are  ADE17, which encodes an isozyme of 5-aminoimidazole-4-carboxamide ribonucleotide transformylase;  DLD3, encoding lactate dehydrogenase;  OAC1, encoding a mitochondrial oxaloacetate transport protein; and  YNL276C, an ORF with an unidentified function.	gene_phenotype
68263	2	333054	5	NULL	NULL	0	NULL	DLD3	GP		encodes					lactate dehydrogenase	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_97_22_12369_s_114	11035792	The remaining four are  ADE17, which encodes an isozyme of 5-aminoimidazole-4-carboxamide ribonucleotide transformylase;  DLD3, encoding lactate dehydrogenase;  OAC1, encoding a mitochondrial oxaloacetate transport protein; and  YNL276C, an ORF with an unidentified function.	gene_phenotype
68264	3	333054	5	NULL	NULL	0	NULL	OAC1	GP		encodes					mitochondrial oxaloacetate transport protein	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_97_22_12369_s_114	11035792	The remaining four are  ADE17, which encodes an isozyme of 5-aminoimidazole-4-carboxamide ribonucleotide transformylase;  DLD3, encoding lactate dehydrogenase;  OAC1, encoding a mitochondrial oxaloacetate transport protein; and  YNL276C, an ORF with an unidentified function.	gene_phenotype
68265	4	333054	5	NULL	NULL	0	NULL	YNL276C	NucleicAcid		is a type of					ORF	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_pnas_97_22_12369_s_114	11035792	The remaining four are  ADE17, which encodes an isozyme of 5-aminoimidazole-4-carboxamide ribonucleotide transformylase;  DLD3, encoding lactate dehydrogenase;  OAC1, encoding a mitochondrial oxaloacetate transport protein; and  YNL276C, an ORF with an unidentified function.	gene_phenotype
68266	1	333055	5	NULL	NULL	0	NULL	Ume6-regulated genes	GP		is induced in		later			meiosis	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_99_21_13431_s_155	12370439	However, several Ume6-regulated genes (mostly of unknown function) appear to be induced later in meiosis (in expression clusters 5-7;  AUT7,  ECM8,  MPC54,  SMA1,  SLZ1,  SSA3,  YBR116C,  YKR005C,  YOL024W,  YOR338W,  YPR027C).	gene_phenotype
68267	1	333056	5	NULL	NULL	0	NULL	Letm1	GP		is transported across					inner mitochondrial membrane	CellComponent				NULL		0	NULL	NULL	NULL	gw70_cellbiol_172_4_553_s_47	16476776	Letm1, Mdm38, and Ylh47 are transported across the inner mitochondrial membrane   The yeast proteins Mdm38 (Yol027c) and Ylh47 (Ypr125w) display significant sequence similarity to the human Letm1 protein ( Fig. 1 A), which has been implicated in WHS.	gene_phenotype
68268	2	333056	5	NULL	NULL	0	NULL	Mdm38	GP		is transported across					inner mitochondrial membrane	CellComponent				NULL		0	NULL	NULL	NULL	gw70_cellbiol_172_4_553_s_47	16476776	Letm1, Mdm38, and Ylh47 are transported across the inner mitochondrial membrane   The yeast proteins Mdm38 (Yol027c) and Ylh47 (Ypr125w) display significant sequence similarity to the human Letm1 protein ( Fig. 1 A), which has been implicated in WHS.	gene_phenotype
68269	3	333056	5	NULL	NULL	0	NULL	Ylh47	GP		is transported across					inner mitochondrial membrane	CellComponent				NULL		0	NULL	NULL	NULL	gw70_cellbiol_172_4_553_s_47	16476776	Letm1, Mdm38, and Ylh47 are transported across the inner mitochondrial membrane   The yeast proteins Mdm38 (Yol027c) and Ylh47 (Ypr125w) display significant sequence similarity to the human Letm1 protein ( Fig. 1 A), which has been implicated in WHS.	gene_phenotype
68273	4	333056	5	NULL	NULL	NULL	NULL	Mdm38 (Yol027c)	GP	sequence of	is similar to		significantly			Letm1 protein	GP	human;;sequence of			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_172_4_553_s_47	16476776	Letm1, Mdm38, and Ylh47 are transported across the inner mitochondrial membrane   The yeast proteins Mdm38 (Yol027c) and Ylh47 (Ypr125w) display significant sequence similarity to the human Letm1 protein ( Fig. 1 A), which has been implicated in WHS.	gene_phenotype
68276	5	333056	5	NULL	NULL	0	NULL	Ylh47 (Ypr125w)	GP	sequence of	is similar to		significantly			Letm1 protein	GP	human;;sequence of			NULL		0	NULL	NULL	NULL	gw70_cellbiol_172_4_553_s_47	16476776	Letm1, Mdm38, and Ylh47 are transported across the inner mitochondrial membrane   The yeast proteins Mdm38 (Yol027c) and Ylh47 (Ypr125w) display significant sequence similarity to the human Letm1 protein ( Fig. 1 A), which has been implicated in WHS.	gene_phenotype
68277	6	333056	5	NULL	NULL	0	NULL	Letm1 protein	GP	human	is implicated in					WHS	MedicalFinding				NULL		0	NULL	NULL	NULL	gw70_cellbiol_172_4_553_s_47	16476776	Letm1, Mdm38, and Ylh47 are transported across the inner mitochondrial membrane   The yeast proteins Mdm38 (Yol027c) and Ylh47 (Ypr125w) display significant sequence similarity to the human Letm1 protein ( Fig. 1 A), which has been implicated in WHS.	gene_phenotype
68278	1	333057	5	NULL	NULL	0	NULL	SGT1	GP		is required for					cell viability	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_4_1_21_s_33	10445024	SGT1 (YOR057w) encodes a 44.9 kDa protein with no obvious homology with other proteins in GenBank, and deletion analysis demonstrated that  SGT1 is required for cell viability (see Experimental Procedures).	gene_phenotype
68280	2	333057	5	NULL	NULL	0	NULL	YOR057w	NucleicAcid		is the locus name of					SGT1	GP				NULL		0	NULL	NULL	NULL	gw60_molcell_4_1_21_s_33	10445024	SGT1 (YOR057w) encodes a 44.9 kDa protein with no obvious homology with other proteins in GenBank, and deletion analysis demonstrated that  SGT1 is required for cell viability (see Experimental Procedures).	gene_phenotype
68281	3	333057	5	NULL	NULL	0	NULL	SGT1	GP		encodes					44.9 kDa protein	GP				NULL		0	NULL	NULL	NULL	gw60_molcell_4_1_21_s_33	10445024	SGT1 (YOR057w) encodes a 44.9 kDa protein with no obvious homology with other proteins in GenBank, and deletion analysis demonstrated that  SGT1 is required for cell viability (see Experimental Procedures).	gene_phenotype
68282	1	333058	5	NULL	NULL	0	NULL	YBT1	GP		is sensitive to		highly			methotrexate	Chemical				NULL		0	NULL	NULL	NULL	gw70_pnas_101_3_793_s_112	14718668	The  YBT1 and  YOR072w heterozygous deletion strains are highly sensitive to methotrexate, and both nonessential gene products may be involved in small molecule transport.	gene_phenotype
68283	2	333058	5	NULL	NULL	0	NULL	YBT1	GP		is involved in		may be			small molecule transport	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_101_3_793_s_112	14718668	The  YBT1 and  YOR072w heterozygous deletion strains are highly sensitive to methotrexate, and both nonessential gene products may be involved in small molecule transport.	gene_phenotype
68284	3	333058	5	NULL	NULL	0	NULL	YOR072w heterozygous deletion strains	NucleicAcid		is sensitive to		highly			methotrexate	Chemical				NULL		0	NULL	NULL	NULL	gw70_pnas_101_3_793_s_112	14718668	The  YBT1 and  YOR072w heterozygous deletion strains are highly sensitive to methotrexate, and both nonessential gene products may be involved in small molecule transport.	gene_phenotype
68285	4	333058	5	NULL	NULL	0	NULL	YOR072w heterozygous deletion strains	NucleicAcid		is involved in		may be			small molecule transport	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_101_3_793_s_112	14718668	The  YBT1 and  YOR072w heterozygous deletion strains are highly sensitive to methotrexate, and both nonessential gene products may be involved in small molecule transport.	gene_phenotype
68286	1	333059	5	NULL	NULL	0	NULL	YOR093C	NucleicAcid	S. cerevisiae 	is a paralog of					CPS1	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_100_10_5980_s_211	12730371	S. cerevisiae YOR093C (a paralog of  CPS1) expression was up-regulated by stress conditions such as heat shock or stationary growth ( ), but functional analysis showed that the yor093c null mutant is viable and did not show an altered phenotype ( ).	gene_phenotype
68287	2	333059	5	NULL	NULL	NULL	NULL	YOR093C	NucleicAcid	S. cerevisiae;;expression of	is up-regulated by					heat shock					NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_10_5980_s_211	12730371	S. cerevisiae YOR093C (a paralog of  CPS1) expression was up-regulated by stress conditions such as heat shock or stationary growth ( ), but functional analysis showed that the yor093c null mutant is viable and did not show an altered phenotype ( ).	gene_phenotype
68288	3	333059	5	NULL	NULL	0	NULL	YOR093C	NucleicAcid	S. cerevisiae;;expression of	is up-regulated by					stationary growth	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_100_10_5980_s_211	12730371	S. cerevisiae YOR093C (a paralog of  CPS1) expression was up-regulated by stress conditions such as heat shock or stationary growth ( ), but functional analysis showed that the yor093c null mutant is viable and did not show an altered phenotype ( ).	gene_phenotype
68289	4	333059	5	NULL	NULL	0	NULL	stationary growth	Process		is a type of					stress condition	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_100_10_5980_s_211	12730371	S. cerevisiae YOR093C (a paralog of  CPS1) expression was up-regulated by stress conditions such as heat shock or stationary growth ( ), but functional analysis showed that the yor093c null mutant is viable and did not show an altered phenotype ( ).	gene_phenotype
68290	5	333059	5	NULL	NULL	0	NULL	heat shock			is a type of					stress condition	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_100_10_5980_s_211	12730371	S. cerevisiae YOR093C (a paralog of  CPS1) expression was up-regulated by stress conditions such as heat shock or stationary growth ( ), but functional analysis showed that the yor093c null mutant is viable and did not show an altered phenotype ( ).	gene_phenotype
68291	6	333059	5	NULL	NULL	0	NULL	yor093c	NucleicAcid	null mutant	does not show					altered phenotype					NULL		0	NULL	NULL	NULL	gw70_pnas_100_10_5980_s_211	12730371	S. cerevisiae YOR093C (a paralog of  CPS1) expression was up-regulated by stress conditions such as heat shock or stationary growth ( ), but functional analysis showed that the yor093c null mutant is viable and did not show an altered phenotype ( ).	gene_phenotype
68292	1	333060	5	NULL	NULL	0	NULL	Leu9p protein	GP		is encoded by					YOR108w gene	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1089_s_135	11158296	However, to date this activity is attributed to a protein termed Leu9p (encoded by the gene  YOR108w), which exhibits high sequence similarity to Leu4p (W. Pelzer, unpublished data).	gene_phenotype
68293	2	333060	5	NULL	NULL	0	NULL	Leu9p protein	GP		is similar to		highly			Leu4p	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1089_s_135	11158296	However, to date this activity is attributed to a protein termed Leu9p (encoded by the gene  YOR108w), which exhibits high sequence similarity to Leu4p (W. Pelzer, unpublished data).	gene_phenotype
68294	1	333061	5	NULL	NULL	0	NULL	SSA4	GP		plays a role in					heat shock					NULL		0	NULL	NULL	NULL	gw60_nature_407_6802_395_s_179	11014197	Of the six transcripts that changed in wild-type cells after 30 min of 500 nM inhibitor treatment, three have no known function (YGR035C, YLR346C, YPL222W) and the others have roles in heat shock ( SSA4), osmotic stress response ( GRE2) and drug resistance ( YOR1).	gene_phenotype
68295	2	333061	5	NULL	NULL	0	NULL	GRE2	GP		plays a role in					osmotic stress response	Process				NULL		0	NULL	NULL	NULL	gw60_nature_407_6802_395_s_179	11014197	Of the six transcripts that changed in wild-type cells after 30 min of 500 nM inhibitor treatment, three have no known function (YGR035C, YLR346C, YPL222W) and the others have roles in heat shock ( SSA4), osmotic stress response ( GRE2) and drug resistance ( YOR1).	gene_phenotype
68296	3	333061	5	NULL	NULL	0	NULL	YOR1	GP		plays a role in					drug resistance	Process				NULL		0	NULL	NULL	NULL	gw60_nature_407_6802_395_s_179	11014197	Of the six transcripts that changed in wild-type cells after 30 min of 500 nM inhibitor treatment, three have no known function (YGR035C, YLR346C, YPL222W) and the others have roles in heat shock ( SSA4), osmotic stress response ( GRE2) and drug resistance ( YOR1).	gene_phenotype
68394	1	333062	5	NULL	NULL	NULL	NULL	YBL083C/ RHK1	GP		plays a role in		likely;;direct			germination	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_24_15530_s_243	12432101	Although a subset of our germination-defective strains derives from aneuploid spores or mutations in the parental diploid, we were successful in identifying genes,  YBL083C/ RHK1 and  PMA2, which likely play a direct role in germination.	gene_phenotype
68395	2	333062	5	NULL	NULL	0	NULL	PMA2	GP		plays a role in		likely;;direct			germination	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_99_24_15530_s_243	12432101	Although a subset of our germination-defective strains derives from aneuploid spores or mutations in the parental diploid, we were successful in identifying genes,  YBL083C/ RHK1 and  PMA2, which likely play a direct role in germination.	gene_phenotype
68403	1	333063	5	NULL	NULL	NULL	NULL	YSA1	GP		encodes					26-kDa ADP-sugar diphosphatase 2	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_42_32925_s_16	10922370	YSA1 (ORF YBR111C) encodes a 26-kDa ADP-sugar diphosphatase 2 ( 1),  NPY1 (ORF YGL067W) encodes a 43.5- kDa NADH diphosphatase 3 ( 6),  PSU1 ( DCP2, ORF YNL118C) encodes a 109-kDa protein with an N-terminal nudix hydrolase domain whose enzymic activity is as yet undetermined but which may be involved in both transcriptional activation ( 7) and mRNA decapping ( 8), while  DDP1 (ORF YOR163W) encodes a 21.5-kDa enzyme that is a member of a unique subgroup of nudix hydrolases that can hydrolyze both diadenosine polyphosphates and non-nudix diphosphoinositol polyphosphate substrates ( 9,  10).	gene_phenotype
68569	2	333063	5	NULL	NULL	0	NULL	ORF YBR111C	NucleicAcid		is the locus name of					YSA1	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_42_32925_s_16	10922370	YSA1 (ORF YBR111C) encodes a 26-kDa ADP-sugar diphosphatase 2 ( 1),  NPY1 (ORF YGL067W) encodes a 43.5- kDa NADH diphosphatase 3 ( 6),  PSU1 ( DCP2, ORF YNL118C) encodes a 109-kDa protein with an N-terminal nudix hydrolase domain whose enzymic activity is as yet undetermined but which may be involved in both transcriptional activation ( 7) and mRNA decapping ( 8), while  DDP1 (ORF YOR163W) encodes a 21.5-kDa enzyme that is a member of a unique subgroup of nudix hydrolases that can hydrolyze both diadenosine polyphosphates and non-nudix diphosphoinositol polyphosphate substrates ( 9,  10).	gene_phenotype
68570	3	333063	5	NULL	NULL	0	NULL	ORF YGL067W	NucleicAcid		is the locus name of					NPY1	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_42_32925_s_16	10922370	YSA1 (ORF YBR111C) encodes a 26-kDa ADP-sugar diphosphatase 2 ( 1),  NPY1 (ORF YGL067W) encodes a 43.5- kDa NADH diphosphatase 3 ( 6),  PSU1 ( DCP2, ORF YNL118C) encodes a 109-kDa protein with an N-terminal nudix hydrolase domain whose enzymic activity is as yet undetermined but which may be involved in both transcriptional activation ( 7) and mRNA decapping ( 8), while  DDP1 (ORF YOR163W) encodes a 21.5-kDa enzyme that is a member of a unique subgroup of nudix hydrolases that can hydrolyze both diadenosine polyphosphates and non-nudix diphosphoinositol polyphosphate substrates ( 9,  10).	gene_phenotype
68571	4	333063	5	NULL	NULL	0	NULL	NPY1	GP		encodes					43.5- kDa NADH diphosphatase 3	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_42_32925_s_16	10922370	YSA1 (ORF YBR111C) encodes a 26-kDa ADP-sugar diphosphatase 2 ( 1),  NPY1 (ORF YGL067W) encodes a 43.5- kDa NADH diphosphatase 3 ( 6),  PSU1 ( DCP2, ORF YNL118C) encodes a 109-kDa protein with an N-terminal nudix hydrolase domain whose enzymic activity is as yet undetermined but which may be involved in both transcriptional activation ( 7) and mRNA decapping ( 8), while  DDP1 (ORF YOR163W) encodes a 21.5-kDa enzyme that is a member of a unique subgroup of nudix hydrolases that can hydrolyze both diadenosine polyphosphates and non-nudix diphosphoinositol polyphosphate substrates ( 9,  10).	gene_phenotype
68572	5	333063	5	NULL	NULL	0	NULL	ORF YNL118C	NucleicAcid		is the locus name of					PSU1	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_42_32925_s_16	10922370	YSA1 (ORF YBR111C) encodes a 26-kDa ADP-sugar diphosphatase 2 ( 1),  NPY1 (ORF YGL067W) encodes a 43.5- kDa NADH diphosphatase 3 ( 6),  PSU1 ( DCP2, ORF YNL118C) encodes a 109-kDa protein with an N-terminal nudix hydrolase domain whose enzymic activity is as yet undetermined but which may be involved in both transcriptional activation ( 7) and mRNA decapping ( 8), while  DDP1 (ORF YOR163W) encodes a 21.5-kDa enzyme that is a member of a unique subgroup of nudix hydrolases that can hydrolyze both diadenosine polyphosphates and non-nudix diphosphoinositol polyphosphate substrates ( 9,  10).	gene_phenotype
68573	6	333063	5	NULL	NULL	0	NULL	PSU1	GP		is a synonym of					DCP2	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_42_32925_s_16	10922370	YSA1 (ORF YBR111C) encodes a 26-kDa ADP-sugar diphosphatase 2 ( 1),  NPY1 (ORF YGL067W) encodes a 43.5- kDa NADH diphosphatase 3 ( 6),  PSU1 ( DCP2, ORF YNL118C) encodes a 109-kDa protein with an N-terminal nudix hydrolase domain whose enzymic activity is as yet undetermined but which may be involved in both transcriptional activation ( 7) and mRNA decapping ( 8), while  DDP1 (ORF YOR163W) encodes a 21.5-kDa enzyme that is a member of a unique subgroup of nudix hydrolases that can hydrolyze both diadenosine polyphosphates and non-nudix diphosphoinositol polyphosphate substrates ( 9,  10).	gene_phenotype
68574	7	333063	5	NULL	NULL	0	NULL	PSU1	GP		encodes					109-kDa protein	GP		N-terminal nudix hydrolase domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_42_32925_s_16	10922370	YSA1 (ORF YBR111C) encodes a 26-kDa ADP-sugar diphosphatase 2 ( 1),  NPY1 (ORF YGL067W) encodes a 43.5- kDa NADH diphosphatase 3 ( 6),  PSU1 ( DCP2, ORF YNL118C) encodes a 109-kDa protein with an N-terminal nudix hydrolase domain whose enzymic activity is as yet undetermined but which may be involved in both transcriptional activation ( 7) and mRNA decapping ( 8), while  DDP1 (ORF YOR163W) encodes a 21.5-kDa enzyme that is a member of a unique subgroup of nudix hydrolases that can hydrolyze both diadenosine polyphosphates and non-nudix diphosphoinositol polyphosphate substrates ( 9,  10).	gene_phenotype
68575	8	333063	5	NULL	NULL	NULL	NULL	109-kDa protein	GP		is involved in		potentially	N-terminal nudix hydrolase domain		transcription	Process	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_42_32925_s_16	10922370	YSA1 (ORF YBR111C) encodes a 26-kDa ADP-sugar diphosphatase 2 ( 1),  NPY1 (ORF YGL067W) encodes a 43.5- kDa NADH diphosphatase 3 ( 6),  PSU1 ( DCP2, ORF YNL118C) encodes a 109-kDa protein with an N-terminal nudix hydrolase domain whose enzymic activity is as yet undetermined but which may be involved in both transcriptional activation ( 7) and mRNA decapping ( 8), while  DDP1 (ORF YOR163W) encodes a 21.5-kDa enzyme that is a member of a unique subgroup of nudix hydrolases that can hydrolyze both diadenosine polyphosphates and non-nudix diphosphoinositol polyphosphate substrates ( 9,  10).	gene_phenotype
68576	9	333063	5	NULL	NULL	NULL	NULL	109-kDa protein	GP		is involved in		potentially	N-terminal nudix hydrolase domain		mRNA	NucleicAcid	decapping of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_42_32925_s_16	10922370	YSA1 (ORF YBR111C) encodes a 26-kDa ADP-sugar diphosphatase 2 ( 1),  NPY1 (ORF YGL067W) encodes a 43.5- kDa NADH diphosphatase 3 ( 6),  PSU1 ( DCP2, ORF YNL118C) encodes a 109-kDa protein with an N-terminal nudix hydrolase domain whose enzymic activity is as yet undetermined but which may be involved in both transcriptional activation ( 7) and mRNA decapping ( 8), while  DDP1 (ORF YOR163W) encodes a 21.5-kDa enzyme that is a member of a unique subgroup of nudix hydrolases that can hydrolyze both diadenosine polyphosphates and non-nudix diphosphoinositol polyphosphate substrates ( 9,  10).	gene_phenotype
68577	10	333063	5	NULL	NULL	0	NULL	ORF YOR163W	NucleicAcid		is the locus name of					DDP1	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_42_32925_s_16	10922370	YSA1 (ORF YBR111C) encodes a 26-kDa ADP-sugar diphosphatase 2 ( 1),  NPY1 (ORF YGL067W) encodes a 43.5- kDa NADH diphosphatase 3 ( 6),  PSU1 ( DCP2, ORF YNL118C) encodes a 109-kDa protein with an N-terminal nudix hydrolase domain whose enzymic activity is as yet undetermined but which may be involved in both transcriptional activation ( 7) and mRNA decapping ( 8), while  DDP1 (ORF YOR163W) encodes a 21.5-kDa enzyme that is a member of a unique subgroup of nudix hydrolases that can hydrolyze both diadenosine polyphosphates and non-nudix diphosphoinositol polyphosphate substrates ( 9,  10).	gene_phenotype
68578	11	333063	5	NULL	NULL	0	NULL	DDP1	GP		encodes					21.5-kDa enzyme	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_42_32925_s_16	10922370	YSA1 (ORF YBR111C) encodes a 26-kDa ADP-sugar diphosphatase 2 ( 1),  NPY1 (ORF YGL067W) encodes a 43.5- kDa NADH diphosphatase 3 ( 6),  PSU1 ( DCP2, ORF YNL118C) encodes a 109-kDa protein with an N-terminal nudix hydrolase domain whose enzymic activity is as yet undetermined but which may be involved in both transcriptional activation ( 7) and mRNA decapping ( 8), while  DDP1 (ORF YOR163W) encodes a 21.5-kDa enzyme that is a member of a unique subgroup of nudix hydrolases that can hydrolyze both diadenosine polyphosphates and non-nudix diphosphoinositol polyphosphate substrates ( 9,  10).	gene_phenotype
68580	12	333063	5	NULL	NULL	0	NULL	21.5-kDa enzyme	GP		is a member of					nudix hydrolases	GP	subgroup of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_42_32925_s_16	10922370	YSA1 (ORF YBR111C) encodes a 26-kDa ADP-sugar diphosphatase 2 ( 1),  NPY1 (ORF YGL067W) encodes a 43.5- kDa NADH diphosphatase 3 ( 6),  PSU1 ( DCP2, ORF YNL118C) encodes a 109-kDa protein with an N-terminal nudix hydrolase domain whose enzymic activity is as yet undetermined but which may be involved in both transcriptional activation ( 7) and mRNA decapping ( 8), while  DDP1 (ORF YOR163W) encodes a 21.5-kDa enzyme that is a member of a unique subgroup of nudix hydrolases that can hydrolyze both diadenosine polyphosphates and non-nudix diphosphoinositol polyphosphate substrates ( 9,  10).	gene_phenotype
68581	13	333063	5	NULL	NULL	0	NULL	nudix hydrolases	GP		hydrolyzes					diadenosine polyphosphates	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_42_32925_s_16	10922370	YSA1 (ORF YBR111C) encodes a 26-kDa ADP-sugar diphosphatase 2 ( 1),  NPY1 (ORF YGL067W) encodes a 43.5- kDa NADH diphosphatase 3 ( 6),  PSU1 ( DCP2, ORF YNL118C) encodes a 109-kDa protein with an N-terminal nudix hydrolase domain whose enzymic activity is as yet undetermined but which may be involved in both transcriptional activation ( 7) and mRNA decapping ( 8), while  DDP1 (ORF YOR163W) encodes a 21.5-kDa enzyme that is a member of a unique subgroup of nudix hydrolases that can hydrolyze both diadenosine polyphosphates and non-nudix diphosphoinositol polyphosphate substrates ( 9,  10).	gene_phenotype
68582	14	333063	5	NULL	NULL	0	NULL	nudix hydrolases	GP		hydrolyzes					non-nudix diphosphoinositol polyphosphate substrates	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_42_32925_s_16	10922370	YSA1 (ORF YBR111C) encodes a 26-kDa ADP-sugar diphosphatase 2 ( 1),  NPY1 (ORF YGL067W) encodes a 43.5- kDa NADH diphosphatase 3 ( 6),  PSU1 ( DCP2, ORF YNL118C) encodes a 109-kDa protein with an N-terminal nudix hydrolase domain whose enzymic activity is as yet undetermined but which may be involved in both transcriptional activation ( 7) and mRNA decapping ( 8), while  DDP1 (ORF YOR163W) encodes a 21.5-kDa enzyme that is a member of a unique subgroup of nudix hydrolases that can hydrolyze both diadenosine polyphosphates and non-nudix diphosphoinositol polyphosphate substrates ( 9,  10).	gene_phenotype
68583	1	333068	5	NULL	NULL	NULL	NULL	GOD1	GP		is a synonym of					SWC4 gene	GP	budding yeast			NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_3_4_976_s_80	15302830	Within this group, 18 clones contained the  S. pombe homolog of the budding yeast gene  SWC4 (YGR002C; this gene has been also named  GOD1 and  EAF2 [ www.yeastgenome.	gene_phenotype
68584	2	333068	5	NULL	NULL	0	NULL	EAF2	GP		is a synonym of					SWC4 gene	GP	budding yeast			NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_3_4_976_s_80	15302830	Within this group, 18 clones contained the  S. pombe homolog of the budding yeast gene  SWC4 (YGR002C; this gene has been also named  GOD1 and  EAF2 [ www.yeastgenome.	gene_phenotype
68585	3	333068	5	NULL	NULL	0	NULL	YGR002C	NucleicAcid		is the locus name of					SWC4 gene	GP	budding yeast			NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_3_4_976_s_80	15302830	Within this group, 18 clones contained the  S. pombe homolog of the budding yeast gene  SWC4 (YGR002C; this gene has been also named  GOD1 and  EAF2 [ www.yeastgenome.	gene_phenotype
68586	1	333071	5	NULL	NULL	NULL	NULL	YIL073C	NucleicAcid		plays a role in		important			spore	Cell	viability of			NULL		NULL	NULL	NULL	NULL	gw60_nature_402_6760_413_s_132	10586881	In any case, our transposon-based approach is an effective means of identifying novel sporulation-induced genes; one gene identified in our screen is  YIL073C, which we found to be important for spore viability and synaptonemal complex formation.	gene_phenotype
68587	2	333071	5	NULL	NULL	0	NULL	YIL073C	NucleicAcid		plays a role in		important			synaptonemal complex	GP	fomation of			NULL		0	NULL	NULL	NULL	gw60_nature_402_6760_413_s_132	10586881	In any case, our transposon-based approach is an effective means of identifying novel sporulation-induced genes; one gene identified in our screen is  YIL073C, which we found to be important for spore viability and synaptonemal complex formation.	gene_phenotype
68588	1	333072	5	NULL	NULL	0	NULL	Afg3p	GP		plays a role in		may			mating	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_99_26_16893_s_172	12482955	YAL004W and  YJL107C are ORFs whose functions are not known; Afg3p, Bud14p, Dia2p, Erg28p, Hmg1p, Hmg2p, Rad6p, Sod1p, and Ste24p were not previously known to be associated with the pheromone-response pathway, but their annotations suggest they may play roles in mating (see SGD,  http://genome-www.	gene_phenotype
68589	2	333072	5	NULL	NULL	0	NULL	Bud14p	GP		plays a role in		may			mating	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_99_26_16893_s_172	12482955	YAL004W and  YJL107C are ORFs whose functions are not known; Afg3p, Bud14p, Dia2p, Erg28p, Hmg1p, Hmg2p, Rad6p, Sod1p, and Ste24p were not previously known to be associated with the pheromone-response pathway, but their annotations suggest they may play roles in mating (see SGD,  http://genome-www.	gene_phenotype
68590	3	333072	5	NULL	NULL	0	NULL	Dia2p	GP		plays a role in		may			mating	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_99_26_16893_s_172	12482955	YAL004W and  YJL107C are ORFs whose functions are not known; Afg3p, Bud14p, Dia2p, Erg28p, Hmg1p, Hmg2p, Rad6p, Sod1p, and Ste24p were not previously known to be associated with the pheromone-response pathway, but their annotations suggest they may play roles in mating (see SGD,  http://genome-www.	gene_phenotype
68591	4	333072	5	NULL	NULL	0	NULL	Erg28p	GP		plays a role in		may			mating	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_99_26_16893_s_172	12482955	YAL004W and  YJL107C are ORFs whose functions are not known; Afg3p, Bud14p, Dia2p, Erg28p, Hmg1p, Hmg2p, Rad6p, Sod1p, and Ste24p were not previously known to be associated with the pheromone-response pathway, but their annotations suggest they may play roles in mating (see SGD,  http://genome-www.	gene_phenotype
68592	5	333072	5	NULL	NULL	0	NULL	Hmg1p	GP		plays a role in		may			mating	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_99_26_16893_s_172	12482955	YAL004W and  YJL107C are ORFs whose functions are not known; Afg3p, Bud14p, Dia2p, Erg28p, Hmg1p, Hmg2p, Rad6p, Sod1p, and Ste24p were not previously known to be associated with the pheromone-response pathway, but their annotations suggest they may play roles in mating (see SGD,  http://genome-www.	gene_phenotype
68593	6	333072	5	NULL	NULL	0	NULL	Hmg2p	GP		plays a role in		may			mating	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_99_26_16893_s_172	12482955	YAL004W and  YJL107C are ORFs whose functions are not known; Afg3p, Bud14p, Dia2p, Erg28p, Hmg1p, Hmg2p, Rad6p, Sod1p, and Ste24p were not previously known to be associated with the pheromone-response pathway, but their annotations suggest they may play roles in mating (see SGD,  http://genome-www.	gene_phenotype
68594	7	333072	5	NULL	NULL	0	NULL	Rad6p	GP		plays a role in		may			mating	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_99_26_16893_s_172	12482955	YAL004W and  YJL107C are ORFs whose functions are not known; Afg3p, Bud14p, Dia2p, Erg28p, Hmg1p, Hmg2p, Rad6p, Sod1p, and Ste24p were not previously known to be associated with the pheromone-response pathway, but their annotations suggest they may play roles in mating (see SGD,  http://genome-www.	gene_phenotype
68595	8	333072	5	NULL	NULL	0	NULL	Sod1p	GP		plays a role in		may			mating	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_99_26_16893_s_172	12482955	YAL004W and  YJL107C are ORFs whose functions are not known; Afg3p, Bud14p, Dia2p, Erg28p, Hmg1p, Hmg2p, Rad6p, Sod1p, and Ste24p were not previously known to be associated with the pheromone-response pathway, but their annotations suggest they may play roles in mating (see SGD,  http://genome-www.	gene_phenotype
68596	9	333072	5	NULL	NULL	0	NULL	Ste24p	GP		plays a role in		may			mating	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_99_26_16893_s_172	12482955	YAL004W and  YJL107C are ORFs whose functions are not known; Afg3p, Bud14p, Dia2p, Erg28p, Hmg1p, Hmg2p, Rad6p, Sod1p, and Ste24p were not previously known to be associated with the pheromone-response pathway, but their annotations suggest they may play roles in mating (see SGD,  http://genome-www.	gene_phenotype
68597	1	333073	5	NULL	NULL	0	NULL	Rad26	GP		is purified from					chromatin	Chromosome				NULL		0	NULL	NULL	NULL	gw60_nature_415_6874_929_s_22	11859374	We found that the slower-migrating protein purified from chromatin was Rad26, whereas the faster-migrating protein was the product of the YKL054C ORF on budding yeast chromosome XI (predicted  Mr 83,900).	gene_phenotype
68598	2	333073	5	NULL	NULL	0	NULL	YKL054C ORF	NucleicAcid	budding yeast	is present in					chromosome XI	Chromosome				NULL		0	NULL	NULL	NULL	gw60_nature_415_6874_929_s_22	11859374	We found that the slower-migrating protein purified from chromatin was Rad26, whereas the faster-migrating protein was the product of the YKL054C ORF on budding yeast chromosome XI (predicted  Mr 83,900).	gene_phenotype
68599	1	333074	5	NULL	NULL	0	NULL	YLR135W	NucleicAcid		is the locus name of					SLX4	GP				NULL		0	NULL	NULL	NULL	gw60_genetics_154_3_1101_s_139	10757756	A strain that is null in both  SGS1 and  SLX4 (YLR135W) is inviable but can be maintained by a copy of  SGS1 on a  URA3-based plasmid.	gene_phenotype
68600	1	333075	5	NULL	NULL	0	NULL	YLR347c	NucleicAcid		is the locus name of					KAP95	GP				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_319_2_349_s_55	15178413	Another known gene  YLR347c ( KAP95) encodes a protein involved in nuclear transport [  28].	gene_phenotype
68601	2	333075	5	NULL	NULL	0	NULL	KAP95	GP		is involved in					nuclear transport	Process				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_319_2_349_s_55	15178413	Another known gene  YLR347c ( KAP95) encodes a protein involved in nuclear transport [  28].	gene_phenotype
68602	1	333076	5	NULL	NULL	0	NULL	Lem3p	GP		interacts with					KAP95	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_38_36041_s_272	12842877	The observation that Lem3p has been shown by high throughput mass spectrometric protein complex identification ( ) to interact with two proteins involved in nuclear import ( YLR347C/ KAP95 and  YJR132W/ NMD5) is consistent with a nuclear function.	gene_phenotype
68603	2	333076	5	NULL	NULL	0	NULL	Lem3p	GP		interacts with					NMD5	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_38_36041_s_272	12842877	The observation that Lem3p has been shown by high throughput mass spectrometric protein complex identification ( ) to interact with two proteins involved in nuclear import ( YLR347C/ KAP95 and  YJR132W/ NMD5) is consistent with a nuclear function.	gene_phenotype
68604	3	333076	5	NULL	NULL	0	NULL	YLR347C	NucleicAcid		is the locus name of					KAP95	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_38_36041_s_272	12842877	The observation that Lem3p has been shown by high throughput mass spectrometric protein complex identification ( ) to interact with two proteins involved in nuclear import ( YLR347C/ KAP95 and  YJR132W/ NMD5) is consistent with a nuclear function.	gene_phenotype
68605	4	333076	5	NULL	NULL	0	NULL	YJR132W	NucleicAcid		is the locus name of					NMD5	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_38_36041_s_272	12842877	The observation that Lem3p has been shown by high throughput mass spectrometric protein complex identification ( ) to interact with two proteins involved in nuclear import ( YLR347C/ KAP95 and  YJR132W/ NMD5) is consistent with a nuclear function.	gene_phenotype
68606	5	333076	5	NULL	NULL	0	NULL	KAP95	GP		is involved in					nuclear import	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_38_36041_s_272	12842877	The observation that Lem3p has been shown by high throughput mass spectrometric protein complex identification ( ) to interact with two proteins involved in nuclear import ( YLR347C/ KAP95 and  YJR132W/ NMD5) is consistent with a nuclear function.	gene_phenotype
68607	6	333076	5	NULL	NULL	0	NULL	NMD5	GP		is involved in					nuclear import	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_38_36041_s_272	12842877	The observation that Lem3p has been shown by high throughput mass spectrometric protein complex identification ( ) to interact with two proteins involved in nuclear import ( YLR347C/ KAP95 and  YJR132W/ NMD5) is consistent with a nuclear function.	gene_phenotype
68608	1	333078	5	NULL	NULL	0	NULL	dopamine transporter gene	GP	inactivation of	leads to					dopamine	Chemical	elevated;;extracellular			NULL	mice	0	NULL	NULL	NULL	gw70_pnas_100_19_11035_s_4	12958210	Here we document that mice with persistently elevated extracellular dopamine, resulting from inactivation of the dopamine transporter gene, sporadically develop severe symptoms of dyskinesia concomitant with apoptotic death of striatal dopamine-responsive gamma-aminobutyric acidergic neurons.	gene_phenotype
68609	2	333078	5	NULL	NULL	0	NULL	statement 1	Process		develops					dyskinesia	MedicalFinding	severe symptoms of			NULL		0	NULL	NULL	NULL	gw70_pnas_100_19_11035_s_4	12958210	Here we document that mice with persistently elevated extracellular dopamine, resulting from inactivation of the dopamine transporter gene, sporadically develop severe symptoms of dyskinesia concomitant with apoptotic death of striatal dopamine-responsive gamma-aminobutyric acidergic neurons.	gene_phenotype
68610	3	333078	5	NULL	NULL	0	NULL	statement 2	Process		is concomitant to					striatal dopamine-responsive gamma-aminobutyric acidergic neurons	Cell	apoptotic death of			NULL		0	NULL	NULL	NULL	gw70_pnas_100_19_11035_s_4	12958210	Here we document that mice with persistently elevated extracellular dopamine, resulting from inactivation of the dopamine transporter gene, sporadically develop severe symptoms of dyskinesia concomitant with apoptotic death of striatal dopamine-responsive gamma-aminobutyric acidergic neurons.	gene_phenotype
68611	1	333080	5	NULL	NULL	0	NULL	Rim15	GP		is a type of					yeast-specific kinase	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_96_24_13603_s_75	10570119	Rim15 is a yeast-specific kinase that is related to  Schizosaccharomyces pombe Cek1, and its similarity to budding yeast YNL161w places it as a distant member of the NDR family kinases.	gene_phenotype
68612	2	333080	5	NULL	NULL	0	NULL	Rim15	GP		is related to					Cek1	GP	Schizosaccharomyces pombe			NULL		0	NULL	NULL	NULL	gw60_pnas_96_24_13603_s_75	10570119	Rim15 is a yeast-specific kinase that is related to  Schizosaccharomyces pombe Cek1, and its similarity to budding yeast YNL161w places it as a distant member of the NDR family kinases.	gene_phenotype
68613	3	333080	5	NULL	NULL	0	NULL	Rim15	GP		is similar to					YNL161w	NucleicAcid	budding yeast			NULL		0	NULL	NULL	NULL	gw60_pnas_96_24_13603_s_75	10570119	Rim15 is a yeast-specific kinase that is related to  Schizosaccharomyces pombe Cek1, and its similarity to budding yeast YNL161w places it as a distant member of the NDR family kinases.	gene_phenotype
68614	4	333080	5	NULL	NULL	0	NULL	Rim15	GP		is a member of					NDR family kinases	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_96_24_13603_s_75	10570119	Rim15 is a yeast-specific kinase that is related to  Schizosaccharomyces pombe Cek1, and its similarity to budding yeast YNL161w places it as a distant member of the NDR family kinases.	gene_phenotype
69420	1	333082	5	NULL	NULL	0	NULL	gene product	GP	putative	is close to					l(3)S027714	NucleicAcid	insertion of			NULL		0	NULL	NULL	NULL	gw60_gene_246_1_157_s_208	10767537	BLASTX searches show that the putative gene product close to the  l(3)S027714 insertion is highly similar to  Xenopus XPMC2 (accession no. U10185), a cell cycle gene that can complement mitotic catastrophe mutations in yeast (  Su and Maller, 1995), and to a hypothetical exonuclease YOL080c of  Saccharomyces cerevisiae (accession no. Z74822).	gene_phenotype
69421	2	333082	5	NULL	NULL	0	NULL	statement 1	GP		is similar to		highly			XPMC2	GP	Xenopus			NULL		0	NULL	NULL	NULL	gw60_gene_246_1_157_s_208	10767537	BLASTX searches show that the putative gene product close to the  l(3)S027714 insertion is highly similar to  Xenopus XPMC2 (accession no. U10185), a cell cycle gene that can complement mitotic catastrophe mutations in yeast (  Su and Maller, 1995), and to a hypothetical exonuclease YOL080c of  Saccharomyces cerevisiae (accession no. Z74822).	gene_phenotype
69422	3	333082	5	NULL	NULL	0	NULL	XPMC2 gene	GP	Xenopus	is a type of					cell cycle gene	GP				NULL		0	NULL	NULL	NULL	gw60_gene_246_1_157_s_208	10767537	BLASTX searches show that the putative gene product close to the  l(3)S027714 insertion is highly similar to  Xenopus XPMC2 (accession no. U10185), a cell cycle gene that can complement mitotic catastrophe mutations in yeast (  Su and Maller, 1995), and to a hypothetical exonuclease YOL080c of  Saccharomyces cerevisiae (accession no. Z74822).	gene_phenotype
69423	4	333082	5	NULL	NULL	0	NULL	XPMC2	GP	Xenopus	complements					mitotic catastrophe mutations	Process				NULL	yeast	0	NULL	NULL	NULL	gw60_gene_246_1_157_s_208	10767537	BLASTX searches show that the putative gene product close to the  l(3)S027714 insertion is highly similar to  Xenopus XPMC2 (accession no. U10185), a cell cycle gene that can complement mitotic catastrophe mutations in yeast (  Su and Maller, 1995), and to a hypothetical exonuclease YOL080c of  Saccharomyces cerevisiae (accession no. Z74822).	gene_phenotype
69424	5	333082	5	NULL	NULL	0	NULL	statement 1	GP		is similar to					YOL080c	NucleicAcid	Saccharomyces cerevisiae			NULL		0	NULL	NULL	NULL	gw60_gene_246_1_157_s_208	10767537	BLASTX searches show that the putative gene product close to the  l(3)S027714 insertion is highly similar to  Xenopus XPMC2 (accession no. U10185), a cell cycle gene that can complement mitotic catastrophe mutations in yeast (  Su and Maller, 1995), and to a hypothetical exonuclease YOL080c of  Saccharomyces cerevisiae (accession no. Z74822).	gene_phenotype
69425	6	333082	5	NULL	NULL	0	NULL	YOL080c	NucleicAcid	Saccharomyces cerevisiae	is a type of					hypothetical exonuclease	GP				NULL		0	NULL	NULL	NULL	gw60_gene_246_1_157_s_208	10767537	BLASTX searches show that the putative gene product close to the  l(3)S027714 insertion is highly similar to  Xenopus XPMC2 (accession no. U10185), a cell cycle gene that can complement mitotic catastrophe mutations in yeast (  Su and Maller, 1995), and to a hypothetical exonuclease YOL080c of  Saccharomyces cerevisiae (accession no. Z74822).	gene_phenotype
68615	1	333083	5	NULL	NULL	NULL	NULL	RNAPII holoenzyme	GP	elongating 	is the product of					YPL086C ORF	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_4_1_123_s_26	10445034	Erdjument-Bromage et al. 1998  ) was used to identify the 60 kDa subunit of elongator and elongating RNAPII holoenzyme as the product of the YPL086C ORF on budding yeast chromosome XVI (predicted  Mr 63 kDa).	gene_phenotype
68616	2	333083	5	NULL	NULL	NULL	NULL	elongator	GP		is the product of			60 kDa subunit		YPL086C ORF	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcell_4_1_123_s_26	10445034	Erdjument-Bromage et al. 1998  ) was used to identify the 60 kDa subunit of elongator and elongating RNAPII holoenzyme as the product of the YPL086C ORF on budding yeast chromosome XVI (predicted  Mr 63 kDa).	gene_phenotype
68617	3	333083	5	NULL	NULL	0	NULL	YPL086C ORF	NucleicAcid		is present in					chromosome XVI	Chromosome	budding yeast			NULL		0	NULL	NULL	NULL	gw60_molcell_4_1_123_s_26	10445034	Erdjument-Bromage et al. 1998  ) was used to identify the 60 kDa subunit of elongator and elongating RNAPII holoenzyme as the product of the YPL086C ORF on budding yeast chromosome XVI (predicted  Mr 63 kDa).	gene_phenotype
68618	1	333084	5	NULL	NULL	0	NULL	YBR156C	NucleicAcid		is the locus name of					SLI15	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_7_1381_s_235	10385519	It has been reported previously that disruption of   YBR156C ( SLI15) leads to loss of cell viability ( 51).	gene_phenotype
68619	2	333084	5	NULL	NULL	0	NULL	SLI15	GP	disruption of	leads to					cell viability	Process	loss of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_145_7_1381_s_235	10385519	It has been reported previously that disruption of   YBR156C ( SLI15) leads to loss of cell viability ( 51).	gene_phenotype
68620	1	333086	5	NULL	NULL	0	NULL	YDR100W	NucleicAcid		plays a role in					vesicular transport	Process				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_5_1163_s_138	11861907	We found that cellular roles could be assigned to four other previously uncharacterized proteins in this way: YDR100W (vesicular transport/membrane fusion), YOR275C (vesicular transport), YIL151C (protein degradation) and SOH1 (Pol II transcription) (data not shown).	gene_phenotype
68621	2	333086	5	NULL	NULL	0	NULL	YDR100W 	NucleicAcid		plays a role in					membrane fusion	Process				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_5_1163_s_138	11861907	We found that cellular roles could be assigned to four other previously uncharacterized proteins in this way: YDR100W (vesicular transport/membrane fusion), YOR275C (vesicular transport), YIL151C (protein degradation) and SOH1 (Pol II transcription) (data not shown).	gene_phenotype
68623	3	333086	5	NULL	NULL	0	NULL	YOR275C	GP		plays a role in					vesicular transport	Process				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_5_1163_s_138	11861907	We found that cellular roles could be assigned to four other previously uncharacterized proteins in this way: YDR100W (vesicular transport/membrane fusion), YOR275C (vesicular transport), YIL151C (protein degradation) and SOH1 (Pol II transcription) (data not shown).	gene_phenotype
68625	4	333086	5	NULL	NULL	0	NULL	YIL151C	GP		plays a role in					protein degradation	Process				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_5_1163_s_138	11861907	We found that cellular roles could be assigned to four other previously uncharacterized proteins in this way: YDR100W (vesicular transport/membrane fusion), YOR275C (vesicular transport), YIL151C (protein degradation) and SOH1 (Pol II transcription) (data not shown).	gene_phenotype
68626	5	333086	5	NULL	NULL	0	NULL	SOH1	GP		plays a role in					Pol II transcription	Process				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_5_1163_s_138	11861907	We found that cellular roles could be assigned to four other previously uncharacterized proteins in this way: YDR100W (vesicular transport/membrane fusion), YOR275C (vesicular transport), YIL151C (protein degradation) and SOH1 (Pol II transcription) (data not shown).	gene_phenotype
68622	1	333087	5	NULL	NULL	0	NULL	Don1p	GP		is encoded by					ORF YDR273w	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_embo_19_14_3657_s_216	10899120	This protein, which we named Don1p (encoded by the ORF YDR273w), is expressed exclusively during meiosis.	gene_phenotype
68624	2	333087	5	NULL	NULL	0	NULL	Don1p	GP		is expressed during		exclusively			meiosis	Process				NULL		0	NULL	NULL	NULL	gw60_embo_19_14_3657_s_216	10899120	This protein, which we named Don1p (encoded by the ORF YDR273w), is expressed exclusively during meiosis.	gene_phenotype
68627	1	333088	5	NULL	NULL	0	NULL	YGR211w	NucleicAcid		is the locus name of					ZPR1 gene	GP	yeast			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_yeast_18_9_11427960_s_3	11427960	Sporulation and tetrad analysis showed that YGR211w,  recently identified as the yeast ZPR1 gene, is an essential gene.	gene_phenotype
68628	1	333089	5	NULL	NULL	0	NULL	YGR277C	NucleicAcid	yeast	is not essential for					viability	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_24_21431_s_168	11923312	The corresponding gene in yeast (YGR277C) is essential for viability, consistent with its expected functional role in the CoA biosynthetic pathway (Saccharomyces Genome Database).	gene_phenotype
68629	2	333089	5	NULL	NULL	0	NULL	YGR277C	NucleicAcid	yeast	plays a role in					CoA biosynthetic pathway	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_24_21431_s_168	11923312	The corresponding gene in yeast (YGR277C) is essential for viability, consistent with its expected functional role in the CoA biosynthetic pathway (Saccharomyces Genome Database).	gene_phenotype
68630	1	333090	5	NULL	NULL	0	NULL	Sl269	GP		complemented by					SPO7	GP				NULL		0	NULL	NULL	NULL	gw60_embo_17_22_6449_s_56	9822591	Sl269 was complemented by  SPO7 (DDBJ/EMBL/GenBank accession No. 349744; SGD accession No. YAL009w) and sl235 by a novel gene (DDBJ/EMBL/GenBank accession No. 500822; SGD accession No. YHR004c) designated  NEM1 (for  nuclear  envelope  morphology; see also below) (Figure  1A).	gene_phenotype
68631	2	333090	5	NULL	NULL	0	NULL	sl235	GP		complemented by					NEM1	GP				NULL		0	NULL	NULL	NULL	gw60_embo_17_22_6449_s_56	9822591	Sl269 was complemented by  SPO7 (DDBJ/EMBL/GenBank accession No. 349744; SGD accession No. YAL009w) and sl235 by a novel gene (DDBJ/EMBL/GenBank accession No. 500822; SGD accession No. YHR004c) designated  NEM1 (for  nuclear  envelope  morphology; see also below) (Figure  1A).	gene_phenotype
68632	3	333090	5	NULL	NULL	0	NULL	NEM1	GP		is					nuclear envelope morphology	GP				NULL		0	NULL	NULL	NULL	gw60_embo_17_22_6449_s_56	9822591	Sl269 was complemented by  SPO7 (DDBJ/EMBL/GenBank accession No. 349744; SGD accession No. YAL009w) and sl235 by a novel gene (DDBJ/EMBL/GenBank accession No. 500822; SGD accession No. YHR004c) designated  NEM1 (for  nuclear  envelope  morphology; see also below) (Figure  1A).	gene_phenotype
68633	1	333091	5	NULL	NULL	0	NULL	NES	AminoAcid		is					nuclear export signal	AminoAcid				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_12_4344_s_28	12773575	We and others have recently shown that the nuclear export signal (NES) for the large subunit is provided by the adapter protein Nmd3p (Yhr170wp).	gene_phenotype
68634	2	333091	5	NULL	NULL	0	NULL	large subunit	GP		is provided by			NES		Nmd3p	GP				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_12_4344_s_28	12773575	We and others have recently shown that the nuclear export signal (NES) for the large subunit is provided by the adapter protein Nmd3p (Yhr170wp).	gene_phenotype
68635	3	333091	5	NULL	NULL	0	NULL	Nmd3p	GP		is a type of					adapter protein	GP				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_12_4344_s_28	12773575	We and others have recently shown that the nuclear export signal (NES) for the large subunit is provided by the adapter protein Nmd3p (Yhr170wp).	gene_phenotype
68636	4	333091	5	NULL	NULL	0	NULL	Yhr170wp	NucleicAcid		is the locus name of					Nmd3p	GP				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_12_4344_s_28	12773575	We and others have recently shown that the nuclear export signal (NES) for the large subunit is provided by the adapter protein Nmd3p (Yhr170wp).	gene_phenotype
68637	1	333093	5	NULL	NULL	NULL	NULL	HUL4 gene	GP	complete disruption of;;yeast	leads to					haploid yeast strains	Cell	viable			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_342_s_9	9858558	In addition, we show that haploid yeast strains bearing complete disruptions of either of two other hect E3 genes of yeast, designated  HUL4 (YJR036C) and  HUL5 (YGL141W), are viable.	gene_phenotype
68638	2	333093	5	NULL	NULL	NULL	NULL	HUL5 gene	GP	complete disruption of;;yeast	leads to					haploid yeast strains	Cell	viable			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_1_342_s_9	9858558	In addition, we show that haploid yeast strains bearing complete disruptions of either of two other hect E3 genes of yeast, designated  HUL4 (YJR036C) and  HUL5 (YGL141W), are viable.	gene_phenotype
68639	3	333093	5	NULL	NULL	0	NULL	HUL4 gene	GP	yeast	is a type of					hect E3 gene		yeast			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_1_342_s_9	9858558	In addition, we show that haploid yeast strains bearing complete disruptions of either of two other hect E3 genes of yeast, designated  HUL4 (YJR036C) and  HUL5 (YGL141W), are viable.	gene_phenotype
68640	4	333093	5	NULL	NULL	0	NULL	HUL5 gene	GP	yeast	is a type of					hect E3 gene	GP	yeast			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_1_342_s_9	9858558	In addition, we show that haploid yeast strains bearing complete disruptions of either of two other hect E3 genes of yeast, designated  HUL4 (YJR036C) and  HUL5 (YGL141W), are viable.	gene_phenotype
68641	5	333093	5	NULL	NULL	0	NULL	YJR036C	NucleicAcid		is the locus name of					HUL4	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_1_342_s_9	9858558	In addition, we show that haploid yeast strains bearing complete disruptions of either of two other hect E3 genes of yeast, designated  HUL4 (YJR036C) and  HUL5 (YGL141W), are viable.	gene_phenotype
68642	6	333093	5	NULL	NULL	0	NULL	YGL141W	NucleicAcid		is the locus name of					HUL5	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_1_342_s_9	9858558	In addition, we show that haploid yeast strains bearing complete disruptions of either of two other hect E3 genes of yeast, designated  HUL4 (YJR036C) and  HUL5 (YGL141W), are viable.	gene_phenotype
68645	1	333094	5	NULL	NULL	0	NULL	YCR023c	NucleicAcid		is a homolog of					multidrug resistance protein	GP				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_21_2_113_s_280	9348664	Proteins with transport related functions are given in  Table 18 and comprise the multidrug resistance protein homologues YCR023c and YJR124c, the  cation/Cl  symporter homologue YBR235w, the Na+/H+ antiporter homologues YDR456w, YJL094c, and YLR318w ( NHA1), the proline/betaine/ -ketoglutarate permease homologue YKL217w ( JEN1), and the anion permease homologue YNL275w.	gene_phenotype
68646	2	333094	5	NULL	NULL	0	NULL	YCR023c	NucleicAcid		plays a role in					transport	Process				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_21_2_113_s_280	9348664	Proteins with transport related functions are given in  Table 18 and comprise the multidrug resistance protein homologues YCR023c and YJR124c, the  cation/Cl  symporter homologue YBR235w, the Na+/H+ antiporter homologues YDR456w, YJL094c, and YLR318w ( NHA1), the proline/betaine/ -ketoglutarate permease homologue YKL217w ( JEN1), and the anion permease homologue YNL275w.	gene_phenotype
68647	3	333094	5	NULL	NULL	0	NULL	YJR124c	NucleicAcid		is a homolog of					multidrug resistance protein	GP				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_21_2_113_s_280	9348664	Proteins with transport related functions are given in  Table 18 and comprise the multidrug resistance protein homologues YCR023c and YJR124c, the  cation/Cl  symporter homologue YBR235w, the Na+/H+ antiporter homologues YDR456w, YJL094c, and YLR318w ( NHA1), the proline/betaine/ -ketoglutarate permease homologue YKL217w ( JEN1), and the anion permease homologue YNL275w.	gene_phenotype
68648	4	333094	5	NULL	NULL	NULL	NULL	YJR124c	NucleicAcid		plays a role in					transport	Process				NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_21_2_113_s_280	9348664	Proteins with transport related functions are given in  Table 18 and comprise the multidrug resistance protein homologues YCR023c and YJR124c, the  cation/Cl  symporter homologue YBR235w, the Na+/H+ antiporter homologues YDR456w, YJL094c, and YLR318w ( NHA1), the proline/betaine/ -ketoglutarate permease homologue YKL217w ( JEN1), and the anion permease homologue YNL275w.	gene_phenotype
68649	5	333094	5	NULL	NULL	NULL	NULL	YBR235w	NucleicAcid		is a homolog of					cation/Cl symporter	GP				NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_21_2_113_s_280	9348664	Proteins with transport related functions are given in  Table 18 and comprise the multidrug resistance protein homologues YCR023c and YJR124c, the  cation/Cl  symporter homologue YBR235w, the Na+/H+ antiporter homologues YDR456w, YJL094c, and YLR318w ( NHA1), the proline/betaine/ -ketoglutarate permease homologue YKL217w ( JEN1), and the anion permease homologue YNL275w.	gene_phenotype
68650	6	333094	5	NULL	NULL	0	NULL	YBR235w	NucleicAcid		plays a role in					transport	Process				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_21_2_113_s_280	9348664	Proteins with transport related functions are given in  Table 18 and comprise the multidrug resistance protein homologues YCR023c and YJR124c, the  cation/Cl  symporter homologue YBR235w, the Na+/H+ antiporter homologues YDR456w, YJL094c, and YLR318w ( NHA1), the proline/betaine/ -ketoglutarate permease homologue YKL217w ( JEN1), and the anion permease homologue YNL275w.	gene_phenotype
68651	7	333094	5	NULL	NULL	0	NULL	YDR456w	NucleicAcid		is a homolog of					Na+/H+ antiporter	GP				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_21_2_113_s_280	9348664	Proteins with transport related functions are given in  Table 18 and comprise the multidrug resistance protein homologues YCR023c and YJR124c, the  cation/Cl  symporter homologue YBR235w, the Na+/H+ antiporter homologues YDR456w, YJL094c, and YLR318w ( NHA1), the proline/betaine/ -ketoglutarate permease homologue YKL217w ( JEN1), and the anion permease homologue YNL275w.	gene_phenotype
68659	8	333094	5	NULL	NULL	0	NULL	YDR456w	NucleicAcid		plays a role in					transport	Process				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_21_2_113_s_280	9348664	Proteins with transport related functions are given in  Table 18 and comprise the multidrug resistance protein homologues YCR023c and YJR124c, the  cation/Cl  symporter homologue YBR235w, the Na+/H+ antiporter homologues YDR456w, YJL094c, and YLR318w ( NHA1), the proline/betaine/ -ketoglutarate permease homologue YKL217w ( JEN1), and the anion permease homologue YNL275w.	gene_phenotype
68660	9	333094	5	NULL	NULL	0	NULL	YJL094c	NucleicAcid		is a homolog of					Na+/H+ antiporter	GP				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_21_2_113_s_280	9348664	Proteins with transport related functions are given in  Table 18 and comprise the multidrug resistance protein homologues YCR023c and YJR124c, the  cation/Cl  symporter homologue YBR235w, the Na+/H+ antiporter homologues YDR456w, YJL094c, and YLR318w ( NHA1), the proline/betaine/ -ketoglutarate permease homologue YKL217w ( JEN1), and the anion permease homologue YNL275w.	gene_phenotype
68661	10	333094	5	NULL	NULL	0	NULL	YJL094c	NucleicAcid		plays a role in					transport	Process				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_21_2_113_s_280	9348664	Proteins with transport related functions are given in  Table 18 and comprise the multidrug resistance protein homologues YCR023c and YJR124c, the  cation/Cl  symporter homologue YBR235w, the Na+/H+ antiporter homologues YDR456w, YJL094c, and YLR318w ( NHA1), the proline/betaine/ -ketoglutarate permease homologue YKL217w ( JEN1), and the anion permease homologue YNL275w.	gene_phenotype
68664	11	333094	5	NULL	NULL	0	NULL	YLR318w	NucleicAcid		is a homolog of					Na+/H+ antiporter	GP				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_21_2_113_s_280	9348664	Proteins with transport related functions are given in  Table 18 and comprise the multidrug resistance protein homologues YCR023c and YJR124c, the  cation/Cl  symporter homologue YBR235w, the Na+/H+ antiporter homologues YDR456w, YJL094c, and YLR318w ( NHA1), the proline/betaine/ -ketoglutarate permease homologue YKL217w ( JEN1), and the anion permease homologue YNL275w.	gene_phenotype
68665	12	333094	5	NULL	NULL	0	NULL	YLR318w	NucleicAcid		plays a role in					transport	Process				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_21_2_113_s_280	9348664	Proteins with transport related functions are given in  Table 18 and comprise the multidrug resistance protein homologues YCR023c and YJR124c, the  cation/Cl  symporter homologue YBR235w, the Na+/H+ antiporter homologues YDR456w, YJL094c, and YLR318w ( NHA1), the proline/betaine/ -ketoglutarate permease homologue YKL217w ( JEN1), and the anion permease homologue YNL275w.	gene_phenotype
68666	13	333094	5	NULL	NULL	0	NULL	YLR318w	NucleicAcid		is the locus name of					NHA1	GP				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_21_2_113_s_280	9348664	Proteins with transport related functions are given in  Table 18 and comprise the multidrug resistance protein homologues YCR023c and YJR124c, the  cation/Cl  symporter homologue YBR235w, the Na+/H+ antiporter homologues YDR456w, YJL094c, and YLR318w ( NHA1), the proline/betaine/ -ketoglutarate permease homologue YKL217w ( JEN1), and the anion permease homologue YNL275w.	gene_phenotype
68667	14	333094	5	NULL	NULL	0	NULL	YKL217w	NucleicAcid		is the locus name of					JEN1	GP				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_21_2_113_s_280	9348664	Proteins with transport related functions are given in  Table 18 and comprise the multidrug resistance protein homologues YCR023c and YJR124c, the  cation/Cl  symporter homologue YBR235w, the Na+/H+ antiporter homologues YDR456w, YJL094c, and YLR318w ( NHA1), the proline/betaine/ -ketoglutarate permease homologue YKL217w ( JEN1), and the anion permease homologue YNL275w.	gene_phenotype
68669	15	333094	5	NULL	NULL	0	NULL	YKL217w	NucleicAcid		is a homolog of					proline/betaine/ -ketoglutarate permease	GP				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_21_2_113_s_280	9348664	Proteins with transport related functions are given in  Table 18 and comprise the multidrug resistance protein homologues YCR023c and YJR124c, the  cation/Cl  symporter homologue YBR235w, the Na+/H+ antiporter homologues YDR456w, YJL094c, and YLR318w ( NHA1), the proline/betaine/ -ketoglutarate permease homologue YKL217w ( JEN1), and the anion permease homologue YNL275w.	gene_phenotype
68670	16	333094	5	NULL	NULL	0	NULL	YKL217w	NucleicAcid		plays a role in					transport	Process				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_21_2_113_s_280	9348664	Proteins with transport related functions are given in  Table 18 and comprise the multidrug resistance protein homologues YCR023c and YJR124c, the  cation/Cl  symporter homologue YBR235w, the Na+/H+ antiporter homologues YDR456w, YJL094c, and YLR318w ( NHA1), the proline/betaine/ -ketoglutarate permease homologue YKL217w ( JEN1), and the anion permease homologue YNL275w.	gene_phenotype
68672	17	333094	5	NULL	NULL	0	NULL	YNL275w	NucleicAcid		is a homolog of					anion permease	GP				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_21_2_113_s_280	9348664	Proteins with transport related functions are given in  Table 18 and comprise the multidrug resistance protein homologues YCR023c and YJR124c, the  cation/Cl  symporter homologue YBR235w, the Na+/H+ antiporter homologues YDR456w, YJL094c, and YLR318w ( NHA1), the proline/betaine/ -ketoglutarate permease homologue YKL217w ( JEN1), and the anion permease homologue YNL275w.	gene_phenotype
68674	18	333094	5	NULL	NULL	0	NULL	YNL275w	NucleicAcid		plays a role in					transport	Process				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_21_2_113_s_280	9348664	Proteins with transport related functions are given in  Table 18 and comprise the multidrug resistance protein homologues YCR023c and YJR124c, the  cation/Cl  symporter homologue YBR235w, the Na+/H+ antiporter homologues YDR456w, YJL094c, and YLR318w ( NHA1), the proline/betaine/ -ketoglutarate permease homologue YKL217w ( JEN1), and the anion permease homologue YNL275w.	gene_phenotype
68679	1	333095	5	NULL	NULL	0	NULL	POX1	GP		encodes					acyl-CoA oxidase	GP				NULL		0	NULL	NULL	NULL	gw60_febslett_487_1_91_s_113	11152891	In five cases, at least two different genes exist in  C. tropicalis because two different RSTs are similar to the same portion of a  S. cerevisiae gene:  POX1 (encoding acyl-CoA oxidase),  CAR1 (arginase)  JEN1 (carboxylic acid transporter protein)  SSU1 (sulfite sensitive protein) and  YMR155w (unknown function).	gene_phenotype
68680	2	333095	5	NULL	NULL	0	NULL	CAR1	GP		encodes					arginase	GP				NULL		0	NULL	NULL	NULL	gw60_febslett_487_1_91_s_113	11152891	In five cases, at least two different genes exist in  C. tropicalis because two different RSTs are similar to the same portion of a  S. cerevisiae gene:  POX1 (encoding acyl-CoA oxidase),  CAR1 (arginase)  JEN1 (carboxylic acid transporter protein)  SSU1 (sulfite sensitive protein) and  YMR155w (unknown function).	gene_phenotype
68681	3	333095	5	NULL	NULL	0	NULL	JEN1 	GP		encodes					carboxylic acid transporter protein	GP				NULL		0	NULL	NULL	NULL	gw60_febslett_487_1_91_s_113	11152891	In five cases, at least two different genes exist in  C. tropicalis because two different RSTs are similar to the same portion of a  S. cerevisiae gene:  POX1 (encoding acyl-CoA oxidase),  CAR1 (arginase)  JEN1 (carboxylic acid transporter protein)  SSU1 (sulfite sensitive protein) and  YMR155w (unknown function).	gene_phenotype
68682	4	333095	5	NULL	NULL	0	NULL	SSU1	GP		encodes					sulfite sensitive protein	GP				NULL		0	NULL	NULL	NULL	gw60_febslett_487_1_91_s_113	11152891	In five cases, at least two different genes exist in  C. tropicalis because two different RSTs are similar to the same portion of a  S. cerevisiae gene:  POX1 (encoding acyl-CoA oxidase),  CAR1 (arginase)  JEN1 (carboxylic acid transporter protein)  SSU1 (sulfite sensitive protein) and  YMR155w (unknown function).	gene_phenotype
68692	1	333097	5	NULL	NULL	0	NULL	delta yol100w	NucleicAcid	disruption of	causes					vegetative growth	Process	very slow			NULL	CEN.PK2 strain	0	NULL	NULL	NULL	abs-batch0680-0699_yeast_14_7_9639312_s_5	9639312	In contrast to the lack of phenotypic consequences of delta yol100w disruptions  in the FY1679 background, in the CEN.PK2 strain even a heterozygous disruption  of the same gene caused striking effects, very slow vegetative growth  and highly impaired sporulation.	gene_phenotype
68693	2	333097	5	NULL	NULL	NULL	NULL	delta yol100w	NucleicAcid	disruption of	causes					sporulation	Process	highly impaired			NULL	CEN.PK2 strain	NULL	NULL	NULL	NULL	abs-batch0680-0699_yeast_14_7_9639312_s_5	9639312	In contrast to the lack of phenotypic consequences of delta yol100w disruptions  in the FY1679 background, in the CEN.PK2 strain even a heterozygous disruption  of the same gene caused striking effects, very slow vegetative growth  and highly impaired sporulation.	gene_phenotype
68695	1	333098	5	NULL	NULL	0	NULL	YOR177c	NucleicAcid		is a synonym of					MPC54	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_99_10_6895_s_78	12011448	YOR177c has since been named  MPC54 and is a meiosis-specific component of the spindle pole body ( 16).	gene_phenotype
68697	2	333098	5	NULL	NULL	0	NULL	MPC54	GP		is a component of		meiosis-specific			spindle pole body	CellComponent				NULL		0	NULL	NULL	NULL	gw60_pnas_99_10_6895_s_78	12011448	YOR177c has since been named  MPC54 and is a meiosis-specific component of the spindle pole body ( 16).	gene_phenotype
68698	1	333100	5	NULL	NULL	0	NULL	YPL120w	NucleicAcid		encodes					Vps30p/Atg6p	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_1_203_s_101	16267277	YPL120w encodes Vps30p/Atg6p, a protein known to be involved in both vesicle-mediated protein traffic to the vacuole and autophagy (Tsukada and Ohsumi, 1993 ; Seaman  et al., 1997 ; Kihara  et al., 2001 ).	gene_phenotype
68699	2	333100	5	NULL	NULL	0	NULL	protein	GP		trafficked to					vacuole	CellComponent				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_1_203_s_101	16267277	YPL120w encodes Vps30p/Atg6p, a protein known to be involved in both vesicle-mediated protein traffic to the vacuole and autophagy (Tsukada and Ohsumi, 1993 ; Seaman  et al., 1997 ; Kihara  et al., 2001 ).	gene_phenotype
68700	3	333100	5	NULL	NULL	0	NULL	vesicle	CellComponent		mediates					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_1_203_s_101	16267277	YPL120w encodes Vps30p/Atg6p, a protein known to be involved in both vesicle-mediated protein traffic to the vacuole and autophagy (Tsukada and Ohsumi, 1993 ; Seaman  et al., 1997 ; Kihara  et al., 2001 ).	gene_phenotype
68701	4	333100	5	NULL	NULL	0	NULL	Vps30p/Atg6p protein	GP		is involved in					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_1_203_s_101	16267277	YPL120w encodes Vps30p/Atg6p, a protein known to be involved in both vesicle-mediated protein traffic to the vacuole and autophagy (Tsukada and Ohsumi, 1993 ; Seaman  et al., 1997 ; Kihara  et al., 2001 ).	gene_phenotype
68702	5	333100	5	NULL	NULL	0	NULL	Vps30p/Atg6p protein	GP		is involved in					autophagy	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_1_203_s_101	16267277	YPL120w encodes Vps30p/Atg6p, a protein known to be involved in both vesicle-mediated protein traffic to the vacuole and autophagy (Tsukada and Ohsumi, 1993 ; Seaman  et al., 1997 ; Kihara  et al., 2001 ).	gene_phenotype
68705	1	333101	5	NULL	NULL	0	NULL	YPR082c	NucleicAcid		is the locus name of					Dib1p	GP				NULL		0	NULL	NULL	NULL	gw60_embo_18_16_4535_s_187	10449419	Dib1p (YPR082c) comprises 142 amino acids and is an orthologue of the  Schizosaccharomyces pombe Dim1p, which previously has been assigned a role in cell cycle progression (Berry and Gould, 1997  ; Berry  et al., 1999  ).	gene_phenotype
68706	2	333101	5	NULL	NULL	0	NULL	Dib1p	GP		is an orthologue of 					Dim1p	GP	Schizosaccharomyces pombe			NULL		0	NULL	NULL	NULL	gw60_embo_18_16_4535_s_187	10449419	Dib1p (YPR082c) comprises 142 amino acids and is an orthologue of the  Schizosaccharomyces pombe Dim1p, which previously has been assigned a role in cell cycle progression (Berry and Gould, 1997  ; Berry  et al., 1999  ).	gene_phenotype
68707	3	333101	5	NULL	NULL	0	NULL	Dim1p	GP		plays a role in					cell cycle	Process	progression of			NULL		0	NULL	NULL	NULL	gw60_embo_18_16_4535_s_187	10449419	Dib1p (YPR082c) comprises 142 amino acids and is an orthologue of the  Schizosaccharomyces pombe Dim1p, which previously has been assigned a role in cell cycle progression (Berry and Gould, 1997  ; Berry  et al., 1999  ).	gene_phenotype
68717	1	333103	5	NULL	NULL	0	NULL	Kap95p	GP	yeast	is similar to					Kap123p	GP	yeast			NULL		0	NULL	NULL	NULL	gw60_cell_89_5_715_s_24	9182759	Comparisons  of the yeast database reveal significant similarities between Kap95p, Kap123p, and two other yeast  ORFs: Pse1p (YMR308c), originally characterized as a gene affecting protein secretion (Chow et al.,  1992   ), and another recently characterized karyopherin beta homolog, Kap104p (YBR017c) (Aitchison et al., 1996   ).	gene_phenotype
68718	2	333103	5	NULL	NULL	0	NULL	Pse1p	GP	yeast	is similar to					Kap104p	GP	yeast			NULL		0	NULL	NULL	NULL	gw60_cell_89_5_715_s_24	9182759	Comparisons  of the yeast database reveal significant similarities between Kap95p, Kap123p, and two other yeast  ORFs: Pse1p (YMR308c), originally characterized as a gene affecting protein secretion (Chow et al.,  1992   ), and another recently characterized karyopherin beta homolog, Kap104p (YBR017c) (Aitchison et al., 1996   ).	gene_phenotype
68719	3	333103	5	NULL	NULL	0	NULL	YMR308c	NucleicAcid	yeast	is the locus name of					Pse1p	GP	yeast			NULL		0	NULL	NULL	NULL	gw60_cell_89_5_715_s_24	9182759	Comparisons  of the yeast database reveal significant similarities between Kap95p, Kap123p, and two other yeast  ORFs: Pse1p (YMR308c), originally characterized as a gene affecting protein secretion (Chow et al.,  1992   ), and another recently characterized karyopherin beta homolog, Kap104p (YBR017c) (Aitchison et al., 1996   ).	gene_phenotype
68720	4	333103	5	NULL	NULL	0	NULL	Pse1p	GP	yeast	affects					protein secretion	Process				NULL		0	NULL	NULL	NULL	gw60_cell_89_5_715_s_24	9182759	Comparisons  of the yeast database reveal significant similarities between Kap95p, Kap123p, and two other yeast  ORFs: Pse1p (YMR308c), originally characterized as a gene affecting protein secretion (Chow et al.,  1992   ), and another recently characterized karyopherin beta homolog, Kap104p (YBR017c) (Aitchison et al., 1996   ).	gene_phenotype
68721	5	333103	5	NULL	NULL	0	NULL	YBR017c	NucleicAcid	yeast	is the locus name of					Kap104p	GP	yeast			NULL		0	NULL	NULL	NULL	gw60_cell_89_5_715_s_24	9182759	Comparisons  of the yeast database reveal significant similarities between Kap95p, Kap123p, and two other yeast  ORFs: Pse1p (YMR308c), originally characterized as a gene affecting protein secretion (Chow et al.,  1992   ), and another recently characterized karyopherin beta homolog, Kap104p (YBR017c) (Aitchison et al., 1996   ).	gene_phenotype
68722	6	333103	5	NULL	NULL	0	NULL	Kap104p	GP	yeast	is a homolog of					karyopherin beta	GP				NULL		0	NULL	NULL	NULL	gw60_cell_89_5_715_s_24	9182759	Comparisons  of the yeast database reveal significant similarities between Kap95p, Kap123p, and two other yeast  ORFs: Pse1p (YMR308c), originally characterized as a gene affecting protein secretion (Chow et al.,  1992   ), and another recently characterized karyopherin beta homolog, Kap104p (YBR017c) (Aitchison et al., 1996   ).	gene_phenotype
68735	1	333104	5	NULL	NULL	0	NULL	Nab2p protein	GP	yeast	interacts with					yTRN	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_7_4141_s_196	9632798	In this study, we show that Nab2p, a yeast protein selected in an exhaustive genomic two-hybrid screen performed with yTRN (also known as YBR017c or Kap104p), specifically interacts with this protein, and we have identified an  S. cerevisiae M9-like nuclear import sequence, NAB35.	gene_phenotype
68736	2	333104	5	NULL	NULL	0	NULL	yTRN	GP		is a synonym of					Kap104p	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_7_4141_s_196	9632798	In this study, we show that Nab2p, a yeast protein selected in an exhaustive genomic two-hybrid screen performed with yTRN (also known as YBR017c or Kap104p), specifically interacts with this protein, and we have identified an  S. cerevisiae M9-like nuclear import sequence, NAB35.	gene_phenotype
68737	3	333104	5	NULL	NULL	0	NULL	YBR017c	NucleicAcid		is the locus name of					yTRN	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_7_4141_s_196	9632798	In this study, we show that Nab2p, a yeast protein selected in an exhaustive genomic two-hybrid screen performed with yTRN (also known as YBR017c or Kap104p), specifically interacts with this protein, and we have identified an  S. cerevisiae M9-like nuclear import sequence, NAB35.	gene_phenotype
68738	4	333104	5	NULL	NULL	NULL	NULL	NAB35	AminoAcid	S. cerevisiae	is a type of					M9-like nuclear import sequence	AminoAcid	S. cerevisiae			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_4141_s_196	9632798	In this study, we show that Nab2p, a yeast protein selected in an exhaustive genomic two-hybrid screen performed with yTRN (also known as YBR017c or Kap104p), specifically interacts with this protein, and we have identified an  S. cerevisiae M9-like nuclear import sequence, NAB35.	gene_phenotype
68739	5	333104	5	NULL	NULL	0	NULL	NAB35	AminoAcid		interacts with					yTRN	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_7_4141_s_196	9632798	In this study, we show that Nab2p, a yeast protein selected in an exhaustive genomic two-hybrid screen performed with yTRN (also known as YBR017c or Kap104p), specifically interacts with this protein, and we have identified an  S. cerevisiae M9-like nuclear import sequence, NAB35.	gene_phenotype
68740	1	333105	5	NULL	NULL	0	NULL	Yhl035cp	NucleicAcid		is a member of					multidrug resistance family/ATP-binding cassette transporter family	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_6_4450_s_214	14534306	Yhl035cp is member of the multidrug resistance family/ATP-binding cassette transporter family and is 64% identical to the yeast bile acid transporter Ybt1p, while the predicted Ybr047wp shows no appreciable similarity with other proteins.	gene_phenotype
68741	2	333105	5	NULL	NULL	NULL	NULL	Yhl035cp	NucleicAcid		is similar to					Ybt1p	GP	yeast			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_6_4450_s_214	14534306	Yhl035cp is member of the multidrug resistance family/ATP-binding cassette transporter family and is 64% identical to the yeast bile acid transporter Ybt1p, while the predicted Ybr047wp shows no appreciable similarity with other proteins.	gene_phenotype
68742	3	333105	5	NULL	NULL	0	NULL	Ybt1p	GP	yeast	is a type of					bile acid transporter	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_6_4450_s_214	14534306	Yhl035cp is member of the multidrug resistance family/ATP-binding cassette transporter family and is 64% identical to the yeast bile acid transporter Ybt1p, while the predicted Ybr047wp shows no appreciable similarity with other proteins.	gene_phenotype
68743	1	333106	5	NULL	NULL	0	NULL	YBR152w	NucleicAcid		activates					suppressor	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_1_577_s_122	9858581	The YEplac112-7A subclone efficiently suppressed the ts192 temperature-sensitive growth defect, confirming that YBR152w contained the suppressor activity (Fig.  1).	gene_phenotype
68744	1	333108	5	NULL	NULL	0	NULL	csm1Delta/csm1Delta	GP		causes					sporulation defect	Process				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_exp-cell-res_294_2_15023545_s_8	15023545	Genetic experiments showed that the two-hybrid isolates  MGS1, CLF1, MCM3, 5, 7 (CDC47), and YDL089w, when overexpressed, partially  suppress the csm1Delta/csm1Delta sporulation defect.	gene_phenotype
68745	2	333108	5	NULL	NULL	0	NULL	MGS1	GP	overexpression of	suppress		partially			statement 1	Process				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_exp-cell-res_294_2_15023545_s_8	15023545	Genetic experiments showed that the two-hybrid isolates  MGS1, CLF1, MCM3, 5, 7 (CDC47), and YDL089w, when overexpressed, partially  suppress the csm1Delta/csm1Delta sporulation defect.	gene_phenotype
68747	3	333108	5	NULL	NULL	0	NULL	CLF1	GP	overexpression of	suppress		partially			statement 1	Process				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_exp-cell-res_294_2_15023545_s_8	15023545	Genetic experiments showed that the two-hybrid isolates  MGS1, CLF1, MCM3, 5, 7 (CDC47), and YDL089w, when overexpressed, partially  suppress the csm1Delta/csm1Delta sporulation defect.	gene_phenotype
68748	4	333108	5	NULL	NULL	0	NULL	MCM3	GP	overexpression of	suppress		partially			statement 1	Process				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_exp-cell-res_294_2_15023545_s_8	15023545	Genetic experiments showed that the two-hybrid isolates  MGS1, CLF1, MCM3, 5, 7 (CDC47), and YDL089w, when overexpressed, partially  suppress the csm1Delta/csm1Delta sporulation defect.	gene_phenotype
68749	5	333108	5	NULL	NULL	0	NULL	CDC47	GP	overexpression of	suppress		partially			statement 1	Process				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_exp-cell-res_294_2_15023545_s_8	15023545	Genetic experiments showed that the two-hybrid isolates  MGS1, CLF1, MCM3, 5, 7 (CDC47), and YDL089w, when overexpressed, partially  suppress the csm1Delta/csm1Delta sporulation defect.	gene_phenotype
68750	6	333108	5	NULL	NULL	0	NULL	YDL089w	GP	overexpression of	suppress		partially			statement 1	Process				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_exp-cell-res_294_2_15023545_s_8	15023545	Genetic experiments showed that the two-hybrid isolates  MGS1, CLF1, MCM3, 5, 7 (CDC47), and YDL089w, when overexpressed, partially  suppress the csm1Delta/csm1Delta sporulation defect.	gene_phenotype
68751	1	333109	5	NULL	NULL	0	NULL	MFB1	GP	yeast	is a type of					mitochondrial morphology gene	GP	yeast			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_9_3756_s_3	16790494	Here, we report the identification of a new yeast mitochondrial morphology gene called  MFB1 (YDR219C).	gene_phenotype
68752	2	333109	5	NULL	NULL	0	NULL	YDR219C	NucleicAcid		is the locus name of					MFB1	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_9_3756_s_3	16790494	Here, we report the identification of a new yeast mitochondrial morphology gene called  MFB1 (YDR219C).	gene_phenotype
68753	1	333110	5	NULL	NULL	0	NULL	Pal1p	GP	budding yeast	is the product of					YDR348c gene	NucleicAcid	budding yeast			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_9_4124_s_390	15975911	As with the budding yeast YDR348c gene product, Pal1p is also detected at the cell division site.	gene_phenotype
68754	2	333110	5	NULL	NULL	NULL	NULL	Pal1p	GP	budding yeast	plays a role in					cell division	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_9_4124_s_390	15975911	As with the budding yeast YDR348c gene product, Pal1p is also detected at the cell division site.	gene_phenotype
68755	1	333111	5	NULL	NULL	0	NULL	Pal1p	GP		interacts with		physically			Sla2p	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_9_4124_s_153	15975911	Pal1p Physically Interacts and Shows Overlapping Localization with Sla2p   The budding yeast Pal1p related protein YDR348c has been shown to copurify with Sla2p in genome-scale proteomic analyses in  S. cerevisiae (Gavin  et al., 2002 ).	gene_phenotype
68756	2	333111	5	NULL	NULL	0	NULL	Pal1p	GP		colocalize with					Sla2p	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_9_4124_s_153	15975911	Pal1p Physically Interacts and Shows Overlapping Localization with Sla2p   The budding yeast Pal1p related protein YDR348c has been shown to copurify with Sla2p in genome-scale proteomic analyses in  S. cerevisiae (Gavin  et al., 2002 ).	gene_phenotype
68757	3	333111	5	NULL	NULL	0	NULL	YDR348c	GP		is a type of					Pal1p related protein	GP	budding yeast			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_9_4124_s_153	15975911	Pal1p Physically Interacts and Shows Overlapping Localization with Sla2p   The budding yeast Pal1p related protein YDR348c has been shown to copurify with Sla2p in genome-scale proteomic analyses in  S. cerevisiae (Gavin  et al., 2002 ).	gene_phenotype
68758	4	333111	5	NULL	NULL	0	NULL	YDR348c	GP		copurify with					Sla2p	GP				NULL	S. cerevisiae	0	NULL	NULL	NULL	gw70_molbiolcell_16_9_4124_s_153	15975911	Pal1p Physically Interacts and Shows Overlapping Localization with Sla2p   The budding yeast Pal1p related protein YDR348c has been shown to copurify with Sla2p in genome-scale proteomic analyses in  S. cerevisiae (Gavin  et al., 2002 ).	gene_phenotype
68759	1	333112	5	NULL	NULL	0	NULL	Pal1p protein	GP	novel	localizes to					growing cell ends	CellComponent				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_9_4124_s_387	15975911	Pal1p, a Novel Protein that Localizes to the Growing Cell Ends and the Division Site   We identified Pal1p as a relative of the budding yeast uncharacterized ORF, YDR348c, which has been shown to localize to the bud neck	gene_phenotype
68760	2	333112	5	NULL	NULL	0	NULL	Pal1p protein	GP	novel	localizes to					division site	CellComponent				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_9_4124_s_387	15975911	Pal1p, a Novel Protein that Localizes to the Growing Cell Ends and the Division Site   We identified Pal1p as a relative of the budding yeast uncharacterized ORF, YDR348c, which has been shown to localize to the bud neck	gene_phenotype
68761	3	333112	5	NULL	NULL	0	NULL	Pal1p protein	GP		is related to					ORF, YDR348c	NucleicAcid	budding yeast;;uncharacterized			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_9_4124_s_387	15975911	Pal1p, a Novel Protein that Localizes to the Growing Cell Ends and the Division Site   We identified Pal1p as a relative of the budding yeast uncharacterized ORF, YDR348c, which has been shown to localize to the bud neck	gene_phenotype
68762	4	333112	5	NULL	NULL	0	NULL	ORF, YDR348c	NucleicAcid	budding yeast;;uncharacterized	localizes to					bud neck	CellComponent				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_9_4124_s_387	15975911	Pal1p, a Novel Protein that Localizes to the Growing Cell Ends and the Division Site   We identified Pal1p as a relative of the budding yeast uncharacterized ORF, YDR348c, which has been shown to localize to the bud neck	gene_phenotype
68763	1	333113	5	NULL	NULL	0	NULL	Pal1p	GP		is a type of					membrane-associated protein	GP	novel			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_9_4124_s_102	15975911	A Novel Membrane-associated Protein, Pal1p, Localizes to the Sites of Active Growth  and Cell Division   We identified a gene,  pal1 ( pears  and  lemons; encoded by SPCP1E11.04c), based on its homology to a novel uncharacterized ORF from budding yeast (YDR348c).	gene_phenotype
68764	2	333113	5	NULL	NULL	0	NULL	Pal1p	GP		localizes to					growth sites	CellComponent	active			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_9_4124_s_102	15975911	A Novel Membrane-associated Protein, Pal1p, Localizes to the Sites of Active Growth  and Cell Division   We identified a gene,  pal1 ( pears  and  lemons; encoded by SPCP1E11.04c), based on its homology to a novel uncharacterized ORF from budding yeast (YDR348c).	gene_phenotype
68765	3	333113	5	NULL	NULL	0	NULL	Pal1p	GP		localizes to					cell division site	CellComponent				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_9_4124_s_102	15975911	A Novel Membrane-associated Protein, Pal1p, Localizes to the Sites of Active Growth  and Cell Division   We identified a gene,  pal1 ( pears  and  lemons; encoded by SPCP1E11.04c), based on its homology to a novel uncharacterized ORF from budding yeast (YDR348c).	gene_phenotype
68766	4	333113	5	NULL	NULL	0	NULL	pal1	GP		is a synonym of					pears and lemons	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_9_4124_s_102	15975911	A Novel Membrane-associated Protein, Pal1p, Localizes to the Sites of Active Growth  and Cell Division   We identified a gene,  pal1 ( pears  and  lemons; encoded by SPCP1E11.04c), based on its homology to a novel uncharacterized ORF from budding yeast (YDR348c).	gene_phenotype
68767	5	333113	5	NULL	NULL	NULL	NULL	pal1	GP		is encoded by					SPCP1E11.04c	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_9_4124_s_102	15975911	A Novel Membrane-associated Protein, Pal1p, Localizes to the Sites of Active Growth  and Cell Division   We identified a gene,  pal1 ( pears  and  lemons; encoded by SPCP1E11.04c), based on its homology to a novel uncharacterized ORF from budding yeast (YDR348c).	gene_phenotype
68768	6	333113	5	NULL	NULL	0	NULL	pal1 gene	GP		is homologous to					ORF YDR348c	NucleicAcid	budding yeast;;uncharacterized			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_9_4124_s_102	15975911	A Novel Membrane-associated Protein, Pal1p, Localizes to the Sites of Active Growth  and Cell Division   We identified a gene,  pal1 ( pears  and  lemons; encoded by SPCP1E11.04c), based on its homology to a novel uncharacterized ORF from budding yeast (YDR348c).	gene_phenotype
68769	1	333115	5	NULL	NULL	0	NULL	Npl6p	GP		interacts with					Rsc8p	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_13_4723_s_291	12052880	As with the genes encoding most other RSC subunits,  NPL6 and  RSC58( YLR033W) are essential for yeast cell viability; moreover, Npl6p has been reported to interact with Rsc8p in yeast two-hybrid assays ( 11).	gene_phenotype
68770	2	333115	5	NULL	NULL	0	NULL	NPL6	GP		is essential for					yeast cells	Cell	viability of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_13_4723_s_291	12052880	As with the genes encoding most other RSC subunits,  NPL6 and  RSC58( YLR033W) are essential for yeast cell viability; moreover, Npl6p has been reported to interact with Rsc8p in yeast two-hybrid assays ( 11).	gene_phenotype
68771	3	333115	5	NULL	NULL	0	NULL	RSC58	GP		is essential for					yeast cells	Cell	viability of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_13_4723_s_291	12052880	As with the genes encoding most other RSC subunits,  NPL6 and  RSC58( YLR033W) are essential for yeast cell viability; moreover, Npl6p has been reported to interact with Rsc8p in yeast two-hybrid assays ( 11).	gene_phenotype
68772	4	333115	5	NULL	NULL	0	NULL	YLR033W	NucleicAcid		is the locus name of					RSC58	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_13_4723_s_291	12052880	As with the genes encoding most other RSC subunits,  NPL6 and  RSC58( YLR033W) are essential for yeast cell viability; moreover, Npl6p has been reported to interact with Rsc8p in yeast two-hybrid assays ( 11).	gene_phenotype
68773	1	333117	5	NULL	NULL	0	NULL	YNL129w protein	GP		does not activate					pyrimidine pathway	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_2_805_s_160	12570998	The inability of the delta urk1delta fur1 double mutant to grow on uracil, uridine, and cytosine shows that no other yeast gene products (e.g., YNL129w protein) have overlapping activity in the pyrimidine pathway.	gene_phenotype
68774	2	333117	5	NULL	NULL	0	NULL	delta urk1delta fur1	GP	double mutant	does not grow on					uracil	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_2_805_s_160	12570998	The inability of the delta urk1delta fur1 double mutant to grow on uracil, uridine, and cytosine shows that no other yeast gene products (e.g., YNL129w protein) have overlapping activity in the pyrimidine pathway.	gene_phenotype
68775	3	333117	5	NULL	NULL	0	NULL	delta urk1delta fur1	GP	double mutant	does not grow on					uridine	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_2_805_s_160	12570998	The inability of the delta urk1delta fur1 double mutant to grow on uracil, uridine, and cytosine shows that no other yeast gene products (e.g., YNL129w protein) have overlapping activity in the pyrimidine pathway.	gene_phenotype
68776	4	333117	5	NULL	NULL	0	NULL	delta urk1delta fur1	GP	double mutant	does not grow on					cytosine	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_2_805_s_160	12570998	The inability of the delta urk1delta fur1 double mutant to grow on uracil, uridine, and cytosine shows that no other yeast gene products (e.g., YNL129w protein) have overlapping activity in the pyrimidine pathway.	gene_phenotype
68777	1	333118	5	NULL	NULL	0	NULL	IMP2	GP		is important for					invasive growth	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_11_1882_s_99	16278455	IMP2,  NCE102,  PUT4,  XBP1, and  YOR161C are important for invasive or pseudohyphal growth ( ,  ).	gene_phenotype
68778	2	333118	5	NULL	NULL	0	NULL	IMP2	GP		is important for					pseudohyphal growth	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_11_1882_s_99	16278455	IMP2,  NCE102,  PUT4,  XBP1, and  YOR161C are important for invasive or pseudohyphal growth ( ,  ).	gene_phenotype
68779	3	333118	5	NULL	NULL	0	NULL	NCE102	GP		is important for					invasive growth	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_11_1882_s_99	16278455	IMP2,  NCE102,  PUT4,  XBP1, and  YOR161C are important for invasive or pseudohyphal growth ( ,  ).	gene_phenotype
68780	4	333118	5	NULL	NULL	0	NULL	NCE102	GP		is important for					pseudohyphal growth	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_11_1882_s_99	16278455	IMP2,  NCE102,  PUT4,  XBP1, and  YOR161C are important for invasive or pseudohyphal growth ( ,  ).	gene_phenotype
68781	5	333118	5	NULL	NULL	0	NULL	PUT4	GP		is important for					invasive growth	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_11_1882_s_99	16278455	IMP2,  NCE102,  PUT4,  XBP1, and  YOR161C are important for invasive or pseudohyphal growth ( ,  ).	gene_phenotype
68782	6	333118	5	NULL	NULL	0	NULL	PUT4	GP		is important for					pseudohyphal growth	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_11_1882_s_99	16278455	IMP2,  NCE102,  PUT4,  XBP1, and  YOR161C are important for invasive or pseudohyphal growth ( ,  ).	gene_phenotype
68783	7	333118	5	NULL	NULL	0	NULL	XBP1	GP		is important for					invasive growth	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_11_1882_s_99	16278455	IMP2,  NCE102,  PUT4,  XBP1, and  YOR161C are important for invasive or pseudohyphal growth ( ,  ).	gene_phenotype
68784	8	333118	5	NULL	NULL	0	NULL	XBP1	GP		is important for					pseudohyphal growth	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_11_1882_s_99	16278455	IMP2,  NCE102,  PUT4,  XBP1, and  YOR161C are important for invasive or pseudohyphal growth ( ,  ).	gene_phenotype
68785	9	333118	5	NULL	NULL	0	NULL	YOR161C	NucleicAcid		is important for					invasive growth	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_11_1882_s_99	16278455	IMP2,  NCE102,  PUT4,  XBP1, and  YOR161C are important for invasive or pseudohyphal growth ( ,  ).	gene_phenotype
68786	10	333118	5	NULL	NULL	0	NULL	YOR161C	NucleicAcid		is important for					pseudohyphal growth	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_11_1882_s_99	16278455	IMP2,  NCE102,  PUT4,  XBP1, and  YOR161C are important for invasive or pseudohyphal growth ( ,  ).	gene_phenotype
68787	11	333118	5	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_11_1882_s_99	16278455	IMP2,  NCE102,  PUT4,  XBP1, and  YOR161C are important for invasive or pseudohyphal growth ( ,  ).	gene_phenotype
68788	12	333118	5	NULL	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_11_1882_s_99	16278455	IMP2,  NCE102,  PUT4,  XBP1, and  YOR161C are important for invasive or pseudohyphal growth ( ,  ).	gene_phenotype
68789	13	333118	5	NULL	NULL	0	NULL	statement 5	Process		is an alternative to					statement 6	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_11_1882_s_99	16278455	IMP2,  NCE102,  PUT4,  XBP1, and  YOR161C are important for invasive or pseudohyphal growth ( ,  ).	gene_phenotype
68790	14	333118	5	NULL	NULL	0	NULL	statement 7	Process		is an alternative to					statement 8	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_11_1882_s_99	16278455	IMP2,  NCE102,  PUT4,  XBP1, and  YOR161C are important for invasive or pseudohyphal growth ( ,  ).	gene_phenotype
68791	15	333118	5	NULL	NULL	0	NULL	statement 9	Process		is an alternative to					statement 10	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_11_1882_s_99	16278455	IMP2,  NCE102,  PUT4,  XBP1, and  YOR161C are important for invasive or pseudohyphal growth ( ,  ).	gene_phenotype
68792	1	333119	5	NULL	NULL	NULL	NULL	apoptosis	Process		is induced by					THG	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_2_569_s_175	16382148	In contrast, coexpression of tTGase suppressed the enhanced sensitivity of GFP-IETD-Smac-transfected cells to THG-induced apoptosis.	gene_phenotype
68793	2	333119	5	NULL	NULL	0	NULL	cells	Cell		transfected with					GFP-IETD-Smac	GP				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_2_569_s_175	16382148	In contrast, coexpression of tTGase suppressed the enhanced sensitivity of GFP-IETD-Smac-transfected cells to THG-induced apoptosis.	gene_phenotype
68794	3	333119	5	NULL	NULL	0	NULL	statement 2	Process		is sensitive to		enhanced			statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_2_569_s_175	16382148	In contrast, coexpression of tTGase suppressed the enhanced sensitivity of GFP-IETD-Smac-transfected cells to THG-induced apoptosis.	gene_phenotype
68795	4	333119	5	NULL	NULL	0	NULL	tTGase	GP	overexpression of	suppress					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_2_569_s_175	16382148	In contrast, coexpression of tTGase suppressed the enhanced sensitivity of GFP-IETD-Smac-transfected cells to THG-induced apoptosis.	gene_phenotype
68796	1	333121	5	NULL	NULL	0	NULL	Sko1 target genes	GP		encodes					Sed1	GP				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_8_1343_s_111	16087739	In particular, Sko1 target genes encode cell wall proteins (Sed1 and Cwp1), vacuolar or cytoplasmic transporters (Stl1, Hxt5, Put4, and Cot1), and confirmed or likely enzymatic activities (Faa1, Sor1, Ald6, and Yor246c).	gene_phenotype
68797	1	333121	5	NULL	NULL	0	NULL	Sko1 target genes	GP		encodes					Sed1	GP				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_8_1343_s_111	16087739	In particular, Sko1 target genes encode cell wall proteins (Sed1 and Cwp1), vacuolar or cytoplasmic transporters (Stl1, Hxt5, Put4, and Cot1), and confirmed or likely enzymatic activities (Faa1, Sor1, Ald6, and Yor246c).	gene_phenotype
68798	2	333121	5	NULL	NULL	0	NULL	Sko1 target genes	GP		encodes					Cwp1	GP				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_8_1343_s_111	16087739	In particular, Sko1 target genes encode cell wall proteins (Sed1 and Cwp1), vacuolar or cytoplasmic transporters (Stl1, Hxt5, Put4, and Cot1), and confirmed or likely enzymatic activities (Faa1, Sor1, Ald6, and Yor246c).	gene_phenotype
68799	3	333121	5	NULL	NULL	0	NULL	Sed1	GP		is a type of					cell wall protein	GP				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_8_1343_s_111	16087739	In particular, Sko1 target genes encode cell wall proteins (Sed1 and Cwp1), vacuolar or cytoplasmic transporters (Stl1, Hxt5, Put4, and Cot1), and confirmed or likely enzymatic activities (Faa1, Sor1, Ald6, and Yor246c).	gene_phenotype
68800	4	333121	5	NULL	NULL	0	NULL	Cwp1	GP		is a type of					cell wall protein	GP				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_8_1343_s_111	16087739	In particular, Sko1 target genes encode cell wall proteins (Sed1 and Cwp1), vacuolar or cytoplasmic transporters (Stl1, Hxt5, Put4, and Cot1), and confirmed or likely enzymatic activities (Faa1, Sor1, Ald6, and Yor246c).	gene_phenotype
68801	5	333121	5	NULL	NULL	0	NULL	Sko1 target genes	GP		encodes					Stl1	GP				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_8_1343_s_111	16087739	In particular, Sko1 target genes encode cell wall proteins (Sed1 and Cwp1), vacuolar or cytoplasmic transporters (Stl1, Hxt5, Put4, and Cot1), and confirmed or likely enzymatic activities (Faa1, Sor1, Ald6, and Yor246c).	gene_phenotype
68802	6	333121	5	NULL	NULL	0	NULL	Stl1	GP		is a type of					vacuolar or cytoplasmic transporter	GP				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_8_1343_s_111	16087739	In particular, Sko1 target genes encode cell wall proteins (Sed1 and Cwp1), vacuolar or cytoplasmic transporters (Stl1, Hxt5, Put4, and Cot1), and confirmed or likely enzymatic activities (Faa1, Sor1, Ald6, and Yor246c).	gene_phenotype
68803	7	333121	5	NULL	NULL	0	NULL	Sko1 target genes	GP		encodes					Hxt5	GP				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_8_1343_s_111	16087739	In particular, Sko1 target genes encode cell wall proteins (Sed1 and Cwp1), vacuolar or cytoplasmic transporters (Stl1, Hxt5, Put4, and Cot1), and confirmed or likely enzymatic activities (Faa1, Sor1, Ald6, and Yor246c).	gene_phenotype
68804	8	333121	5	NULL	NULL	0	NULL	Hxt5	GP		is a type of					vacuolar or cytoplasmic transporter	GP				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_8_1343_s_111	16087739	In particular, Sko1 target genes encode cell wall proteins (Sed1 and Cwp1), vacuolar or cytoplasmic transporters (Stl1, Hxt5, Put4, and Cot1), and confirmed or likely enzymatic activities (Faa1, Sor1, Ald6, and Yor246c).	gene_phenotype
68805	9	333121	5	NULL	NULL	0	NULL	Sko1 target genes	GP		encodes					Put4	GP				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_8_1343_s_111	16087739	In particular, Sko1 target genes encode cell wall proteins (Sed1 and Cwp1), vacuolar or cytoplasmic transporters (Stl1, Hxt5, Put4, and Cot1), and confirmed or likely enzymatic activities (Faa1, Sor1, Ald6, and Yor246c).	gene_phenotype
68806	10	333121	5	NULL	NULL	0	NULL	Put4	GP		is a type of					vacuolar or cytoplasmic transporter	GP				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_8_1343_s_111	16087739	In particular, Sko1 target genes encode cell wall proteins (Sed1 and Cwp1), vacuolar or cytoplasmic transporters (Stl1, Hxt5, Put4, and Cot1), and confirmed or likely enzymatic activities (Faa1, Sor1, Ald6, and Yor246c).	gene_phenotype
68807	11	333121	5	NULL	NULL	0	NULL	Sko1 target genes	GP		encodes					Cot1	GP				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_8_1343_s_111	16087739	In particular, Sko1 target genes encode cell wall proteins (Sed1 and Cwp1), vacuolar or cytoplasmic transporters (Stl1, Hxt5, Put4, and Cot1), and confirmed or likely enzymatic activities (Faa1, Sor1, Ald6, and Yor246c).	gene_phenotype
68808	12	333121	5	NULL	NULL	0	NULL	Cot1	GP		is a type of					vacuolar or cytoplasmic transporter	GP				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_8_1343_s_111	16087739	In particular, Sko1 target genes encode cell wall proteins (Sed1 and Cwp1), vacuolar or cytoplasmic transporters (Stl1, Hxt5, Put4, and Cot1), and confirmed or likely enzymatic activities (Faa1, Sor1, Ald6, and Yor246c).	gene_phenotype
68809	13	333121	5	NULL	NULL	0	NULL	Sko1 target genes	GP		encodes					Faa1	GP				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_8_1343_s_111	16087739	In particular, Sko1 target genes encode cell wall proteins (Sed1 and Cwp1), vacuolar or cytoplasmic transporters (Stl1, Hxt5, Put4, and Cot1), and confirmed or likely enzymatic activities (Faa1, Sor1, Ald6, and Yor246c).	gene_phenotype
68810	14	333121	5	NULL	NULL	0	NULL	Sko1 target genes	GP		encodes					Sor1	GP				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_8_1343_s_111	16087739	In particular, Sko1 target genes encode cell wall proteins (Sed1 and Cwp1), vacuolar or cytoplasmic transporters (Stl1, Hxt5, Put4, and Cot1), and confirmed or likely enzymatic activities (Faa1, Sor1, Ald6, and Yor246c).	gene_phenotype
68811	15	333121	5	NULL	NULL	0	NULL	Sko1 target genes	GP		encodes					Ald6	GP				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_8_1343_s_111	16087739	In particular, Sko1 target genes encode cell wall proteins (Sed1 and Cwp1), vacuolar or cytoplasmic transporters (Stl1, Hxt5, Put4, and Cot1), and confirmed or likely enzymatic activities (Faa1, Sor1, Ald6, and Yor246c).	gene_phenotype
68812	16	333121	5	NULL	NULL	0	NULL	Sko1 target genes	GP		encodes					Yor246c	GP				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_8_1343_s_111	16087739	In particular, Sko1 target genes encode cell wall proteins (Sed1 and Cwp1), vacuolar or cytoplasmic transporters (Stl1, Hxt5, Put4, and Cot1), and confirmed or likely enzymatic activities (Faa1, Sor1, Ald6, and Yor246c).	gene_phenotype
68813	16	333121	5	NULL	NULL	0	NULL	Sko1 target genes	GP		encodes					Yor246c	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_8_1343_s_111	16087739	In particular, Sko1 target genes encode cell wall proteins (Sed1 and Cwp1), vacuolar or cytoplasmic transporters (Stl1, Hxt5, Put4, and Cot1), and confirmed or likely enzymatic activities (Faa1, Sor1, Ald6, and Yor246c).	gene_phenotype
68815	1	333122	5	NULL	NULL	0	NULL	Zds2	GP		interacts with					Cdc11	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_154_3_549_s_202	11489916	Zds2 also interacts with the septin Cdc11, a sporulation-specific protein, Spr6 ( Kallal et al., 1990), and three proteins of unknown function, Yer124c, Yal004w, and Yel023c.	gene_phenotype
68816	2	333122	5	NULL	NULL	0	NULL	Cdc11	GP		is a type of					septin	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_154_3_549_s_202	11489916	Zds2 also interacts with the septin Cdc11, a sporulation-specific protein, Spr6 ( Kallal et al., 1990), and three proteins of unknown function, Yer124c, Yal004w, and Yel023c.	gene_phenotype
68817	3	333122	5	NULL	NULL	0	NULL	Zds2	GP		interacts with					Spr6	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_154_3_549_s_202	11489916	Zds2 also interacts with the septin Cdc11, a sporulation-specific protein, Spr6 ( Kallal et al., 1990), and three proteins of unknown function, Yer124c, Yal004w, and Yel023c.	gene_phenotype
68818	4	333122	5	NULL	NULL	0	NULL	Spr6	GP		is a type of					sporulation-specific protein	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_154_3_549_s_202	11489916	Zds2 also interacts with the septin Cdc11, a sporulation-specific protein, Spr6 ( Kallal et al., 1990), and three proteins of unknown function, Yer124c, Yal004w, and Yel023c.	gene_phenotype
68819	5	333122	5	NULL	NULL	0	NULL	Zds2	GP		interacts with					Yer124c	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_154_3_549_s_202	11489916	Zds2 also interacts with the septin Cdc11, a sporulation-specific protein, Spr6 ( Kallal et al., 1990), and three proteins of unknown function, Yer124c, Yal004w, and Yel023c.	gene_phenotype
68820	6	333122	5	NULL	NULL	0	NULL	Zds2	GP		interacts with					Yal004w	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_154_3_549_s_202	11489916	Zds2 also interacts with the septin Cdc11, a sporulation-specific protein, Spr6 ( Kallal et al., 1990), and three proteins of unknown function, Yer124c, Yal004w, and Yel023c.	gene_phenotype
68821	7	333122	5	NULL	NULL	0	NULL	Zds2	GP		interacts with					Yel023c	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_154_3_549_s_202	11489916	Zds2 also interacts with the septin Cdc11, a sporulation-specific protein, Spr6 ( Kallal et al., 1990), and three proteins of unknown function, Yer124c, Yal004w, and Yel023c.	gene_phenotype
68822	1	333123	5	NULL	NULL	0	NULL	YAL022c	NucleicAcid		is a type of					open reading frame	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_34_25931_s_84	10827169	FUN26, the protein of unknown function predicted from the YAL022c open reading frame, has limited (~18%) amino acid sequence identity with members of the ENT family of nucleoside transporters.	gene_phenotype
68823	2	333123	5	NULL	NULL	0	NULL	YAL022c	NucleicAcid		encodes		possibly			FUN26 protein	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_34_25931_s_84	10827169	FUN26, the protein of unknown function predicted from the YAL022c open reading frame, has limited (~18%) amino acid sequence identity with members of the ENT family of nucleoside transporters.	gene_phenotype
68824	3	333123	5	NULL	NULL	0	NULL	FUN26 protein	GP		is similar to					ENT family of nucleoside transporters	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_34_25931_s_84	10827169	FUN26, the protein of unknown function predicted from the YAL022c open reading frame, has limited (~18%) amino acid sequence identity with members of the ENT family of nucleoside transporters.	gene_phenotype
68825	1	333129	5	NULL	NULL	0	NULL	PBP2	GP	deletion of	leads to					growth	Process	decrease in;;rate of			NULL		0	NULL	NULL	NULL	gw60_currbiol_11_13_1001_s_144	11470404	Deletion of a third gene( YBR233W/ PBP2) also led to a decreased growth rate and caused a more modest meiotic chromosome missegregation, resulting in a spore viability of 5%.	gene_phenotype
68826	2	333129	5	NULL	NULL	0	NULL	PBP2	GP	deletion of	leads to					meiotic chromosome missegregation	Process				NULL		0	NULL	NULL	NULL	gw60_currbiol_11_13_1001_s_144	11470404	Deletion of a third gene( YBR233W/ PBP2) also led to a decreased growth rate and caused a more modest meiotic chromosome missegregation, resulting in a spore viability of 5%.	gene_phenotype
68827	3	333129	5	NULL	NULL	0	NULL	YBR233W	NucleicAcid		is the locus name of					PBP2	GP				NULL		0	NULL	NULL	NULL	gw60_currbiol_11_13_1001_s_144	11470404	Deletion of a third gene( YBR233W/ PBP2) also led to a decreased growth rate and caused a more modest meiotic chromosome missegregation, resulting in a spore viability of 5%.	gene_phenotype
68828	1	333130	5	NULL	NULL	NULL	NULL	YDL033c	NucleicAcid		is involved in		may be			tRNAs	NucleicAcid	2-thio modification of;;mt			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_2_1613_s_146	15509579	Thus, to examine the involvement of YDL033c in the 2-thio modification of the mt tRNAs for Lys, Glu, and Gln and the cytosolic tRNALys, total RNAs obtained from the YDL033c-deletion strain were subjected to polyacrylamide gel electrophoresis containing ( N-acryloylamino)phenylmercuric chloride (APM) combined with Northern blotting ( ,  ) (see "Experimental Procedures"`) ( Fig. 2).	gene_phenotype
68829	2	333130	5	NULL	NULL	0	NULL	YDL033c	NucleicAcid		is involved in		may be			tRNALys	NucleicAcid	2-thio modification of;;cytosolic			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_2_1613_s_146	15509579	Thus, to examine the involvement of YDL033c in the 2-thio modification of the mt tRNAs for Lys, Glu, and Gln and the cytosolic tRNALys, total RNAs obtained from the YDL033c-deletion strain were subjected to polyacrylamide gel electrophoresis containing ( N-acryloylamino)phenylmercuric chloride (APM) combined with Northern blotting ( ,  ) (see "Experimental Procedures"`) ( Fig. 2).	gene_phenotype
68830	1	333131	5	NULL	NULL	0	NULL	YLL034C	NucleicAcid		is a type of					mating pheromone	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_26_26830_s_237	15078868	Interestingly, most of the genes affected by  san1delta are affected transcriptionally by mating pheromone ( YLL034C, HSP12, YDL037C, and  YLL053C; see Ref.  ) or are involved in the pheromone response pathway ( PRM7).	gene_phenotype
68831	2	333131	5	NULL	NULL	0	NULL	HSP12	NucleicAcid		is a type of					mating pheromone	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_26_26830_s_237	15078868	Interestingly, most of the genes affected by  san1delta are affected transcriptionally by mating pheromone ( YLL034C, HSP12, YDL037C, and  YLL053C; see Ref.  ) or are involved in the pheromone response pathway ( PRM7).	gene_phenotype
68832	3	333131	5	NULL	NULL	0	NULL	YDL037C	NucleicAcid		is a type of					mating pheromone	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_26_26830_s_237	15078868	Interestingly, most of the genes affected by  san1delta are affected transcriptionally by mating pheromone ( YLL034C, HSP12, YDL037C, and  YLL053C; see Ref.  ) or are involved in the pheromone response pathway ( PRM7).	gene_phenotype
68833	4	333131	5	NULL	NULL	0	NULL	YLL053C	NucleicAcid		is a type of					mating pheromone	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_26_26830_s_237	15078868	Interestingly, most of the genes affected by  san1delta are affected transcriptionally by mating pheromone ( YLL034C, HSP12, YDL037C, and  YLL053C; see Ref.  ) or are involved in the pheromone response pathway ( PRM7).	gene_phenotype
68834	5	333131	5	NULL	NULL	0	NULL	PRM7	Process		is					pheromone response pathway	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_26_26830_s_237	15078868	Interestingly, most of the genes affected by  san1delta are affected transcriptionally by mating pheromone ( YLL034C, HSP12, YDL037C, and  YLL053C; see Ref.  ) or are involved in the pheromone response pathway ( PRM7).	gene_phenotype
68835	7	333131	5	NULL	NULL	NULL	NULL	statement 1	GP		affects		transcriptionaly			statement 6	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_26_26830_s_237	15078868	Interestingly, most of the genes affected by  san1delta are affected transcriptionally by mating pheromone ( YLL034C, HSP12, YDL037C, and  YLL053C; see Ref.  ) or are involved in the pheromone response pathway ( PRM7).	gene_phenotype
68836	6	333131	5	NULL	NULL	0	NULL	genes	GP		is affected by					san1delta	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_26_26830_s_237	15078868	Interestingly, most of the genes affected by  san1delta are affected transcriptionally by mating pheromone ( YLL034C, HSP12, YDL037C, and  YLL053C; see Ref.  ) or are involved in the pheromone response pathway ( PRM7).	gene_phenotype
68837	8	333131	5	NULL	NULL	0	NULL	statement 2	GP		affects		transcriptionaly			statement 6	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_26_26830_s_237	15078868	Interestingly, most of the genes affected by  san1delta are affected transcriptionally by mating pheromone ( YLL034C, HSP12, YDL037C, and  YLL053C; see Ref.  ) or are involved in the pheromone response pathway ( PRM7).	gene_phenotype
68838	9	333131	5	NULL	NULL	0	NULL	statement 3	GP		affects		transcriptionaly			statement 6	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_26_26830_s_237	15078868	Interestingly, most of the genes affected by  san1delta are affected transcriptionally by mating pheromone ( YLL034C, HSP12, YDL037C, and  YLL053C; see Ref.  ) or are involved in the pheromone response pathway ( PRM7).	gene_phenotype
68839	10	333131	5	NULL	NULL	0	NULL	statement 4	GP		affects		transcriptionaly			statement 6	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_26_26830_s_237	15078868	Interestingly, most of the genes affected by  san1delta are affected transcriptionally by mating pheromone ( YLL034C, HSP12, YDL037C, and  YLL053C; see Ref.  ) or are involved in the pheromone response pathway ( PRM7).	gene_phenotype
68840	11	333131	5	NULL	NULL	0	NULL	statement 6	GP		is involved in		tr			PRM7	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_26_26830_s_237	15078868	Interestingly, most of the genes affected by  san1delta are affected transcriptionally by mating pheromone ( YLL034C, HSP12, YDL037C, and  YLL053C; see Ref.  ) or are involved in the pheromone response pathway ( PRM7).	gene_phenotype
68841	1	333132	5	NULL	NULL	0	NULL	YDL105w	NucleicAcid	budding yeast	is a component of					SMC5+6 complex	GP	yeast			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_11_4866_s_143	15331764	Notably, budding yeast YDL105w was recently identified in a high throughput mass spectrometry and two-hybrid screen as a component of the yeast SMC5+6 complex (Hazbun  et al., 2003 ).	gene_phenotype
68842	1	333134	5	NULL	NULL	NULL	NULL	SEP7/SHS1	GP	deletion of	does not effect					sporulation	Process				NULL		NULL	NULL	NULL	NULL	gw60_genetics_163_1_47_s_200	12586695	Deletions of genes  SEP7/SHS1,  PHO91,  YDL121C, and  YJR003C had little or no effect on sporulation in our hands.	gene_phenotype
68843	2	333134	5	NULL	NULL	0	NULL	PHO91	GP	deletion of	does not effect					sporulation	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_163_1_47_s_200	12586695	Deletions of genes  SEP7/SHS1,  PHO91,  YDL121C, and  YJR003C had little or no effect on sporulation in our hands.	gene_phenotype
68844	3	333134	5	NULL	NULL	0	NULL	YDL121C	NucleicAcid	deletion of	does not effect					sporulation	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_163_1_47_s_200	12586695	Deletions of genes  SEP7/SHS1,  PHO91,  YDL121C, and  YJR003C had little or no effect on sporulation in our hands.	gene_phenotype
68845	4	333134	5	NULL	NULL	0	NULL	YJR003C	NucleicAcid	deletion of	does not effect					sporulation	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_163_1_47_s_200	12586695	Deletions of genes  SEP7/SHS1,  PHO91,  YDL121C, and  YJR003C had little or no effect on sporulation in our hands.	gene_phenotype
68846	1	333135	5	NULL	NULL	0	NULL	SWR1	GP		is a synonym of					YDR334W	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_47_44870_s_111	12244097	The name  SWR1 was proposed for  YDR334W after its identification in a genetic screen for suppressors of yeast impaired in nuclear transport.	gene_phenotype
68847	3	333135	5	NULL	NULL	0	NULL	SWR1	GP		suppress					statement 2	Cell				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_47_44870_s_111	12244097	The name  SWR1 was proposed for  YDR334W after its identification in a genetic screen for suppressors of yeast impaired in nuclear transport.	gene_phenotype
68848	2	333135	5	NULL	NULL	0	NULL	yeast	Cell		impaired in					nuclear transport	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_47_44870_s_111	12244097	The name  SWR1 was proposed for  YDR334W after its identification in a genetic screen for suppressors of yeast impaired in nuclear transport.	gene_phenotype
68849	1	333136	5	NULL	NULL	0	NULL	YER074W-A	NucleicAcid		suppress					yip1-4 Strain	Cell				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_4_1673_s_87	15659647	Identification of YER074W-A as a Novel Multicopy Suppressor of the yip1-4 Strain   Our recent biochemical, genetic, and morphological studies of Yip1p function in protein transport between the ER and the Golgi complex led to the finding that Yip1p plays a critical role in COPII vesicle biogenesis (Heidtman  et al., 2003 ).	gene_phenotype
68850	2	333136	5	NULL	NULL	0	NULL	Yip1p	GP		plays a role in		critical			COPII vesicle	CellComponent	biogenesis of			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_4_1673_s_87	15659647	Identification of YER074W-A as a Novel Multicopy Suppressor of the yip1-4 Strain   Our recent biochemical, genetic, and morphological studies of Yip1p function in protein transport between the ER and the Golgi complex led to the finding that Yip1p plays a critical role in COPII vesicle biogenesis (Heidtman  et al., 2003 ).	gene_phenotype
68851	1	333137	5	NULL	NULL	0	NULL	MEC1	GP	overexpression of	causes					silencing defect	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_158_1_145_s_100	11333225	We constructed a plasmid (pRC12) that had one of these ORFs (YER120W,  SCS2) and showed that this plasmid suppressed the silencing defect caused by  MEC1 overexpression ( Fig 1A).	gene_phenotype
68852	2	333137	5	NULL	NULL	0	NULL	plasmid (pRC12)	CellComponent		suppress					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_158_1_145_s_100	11333225	We constructed a plasmid (pRC12) that had one of these ORFs (YER120W,  SCS2) and showed that this plasmid suppressed the silencing defect caused by  MEC1 overexpression ( Fig 1A).	gene_phenotype
68853	3	333137	5	NULL	NULL	0	NULL	plasmid (pRC12)	CellComponent		contains					YER120W	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_genetics_158_1_145_s_100	11333225	We constructed a plasmid (pRC12) that had one of these ORFs (YER120W,  SCS2) and showed that this plasmid suppressed the silencing defect caused by  MEC1 overexpression ( Fig 1A).	gene_phenotype
68854	4	333137	5	NULL	NULL	0	NULL	plasmid (pRC12)	CellComponent		contains					SCS2	GP				NULL		0	NULL	NULL	NULL	gw60_genetics_158_1_145_s_100	11333225	We constructed a plasmid (pRC12) that had one of these ORFs (YER120W,  SCS2) and showed that this plasmid suppressed the silencing defect caused by  MEC1 overexpression ( Fig 1A).	gene_phenotype
68855	5	333137	5	NULL	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_158_1_145_s_100	11333225	We constructed a plasmid (pRC12) that had one of these ORFs (YER120W,  SCS2) and showed that this plasmid suppressed the silencing defect caused by  MEC1 overexpression ( Fig 1A).	gene_phenotype
68856	1	333139	5	NULL	NULL	NULL	NULL	YGL175C	NucleicAcid		is an ORF of					SAE2/ COM1	GP	full length			NULL		NULL	NULL	NULL	NULL	gw60_genetics_158_1_109_s_107	11333222	Further subcloning and complementation indicated that plasmids harboring the full-length  SAE2/ COM1 ORF alone (YGL175C) were sufficient for full complementation of the sporulation, MMS sensitivity, and mutator phenotypes (data not shown).	gene_phenotype
68857	2	333139	5	NULL	NULL	NULL	NULL	plasmids	CellComponent		harbor		alone			statement 1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genetics_158_1_109_s_107	11333222	Further subcloning and complementation indicated that plasmids harboring the full-length  SAE2/ COM1 ORF alone (YGL175C) were sufficient for full complementation of the sporulation, MMS sensitivity, and mutator phenotypes (data not shown).	gene_phenotype
68858	3	333139	5	NULL	NULL	NULL	NULL	statement 2	CellComponent		is sufficient for					sporulation	Process	full complementation of 			NULL		NULL	NULL	NULL	NULL	gw60_genetics_158_1_109_s_107	11333222	Further subcloning and complementation indicated that plasmids harboring the full-length  SAE2/ COM1 ORF alone (YGL175C) were sufficient for full complementation of the sporulation, MMS sensitivity, and mutator phenotypes (data not shown).	gene_phenotype
68859	4	333139	5	NULL	NULL	NULL	NULL	statement 3	CellComponent		is sufficient for					MMS sensitivity	Process				NULL		NULL	NULL	NULL	NULL	gw60_genetics_158_1_109_s_107	11333222	Further subcloning and complementation indicated that plasmids harboring the full-length  SAE2/ COM1 ORF alone (YGL175C) were sufficient for full complementation of the sporulation, MMS sensitivity, and mutator phenotypes (data not shown).	gene_phenotype
68860	5	333139	5	NULL	NULL	NULL	NULL	statement 3	CellComponent		is sufficient for					mutator phenotypes					NULL		NULL	NULL	NULL	NULL	gw60_genetics_158_1_109_s_107	11333222	Further subcloning and complementation indicated that plasmids harboring the full-length  SAE2/ COM1 ORF alone (YGL175C) were sufficient for full complementation of the sporulation, MMS sensitivity, and mutator phenotypes (data not shown).	gene_phenotype
68861	1	333140	5	NULL	NULL	0	NULL	YGL175C	NucleicAcid		is an ORF of					SAE2/ COM1 	GP	full length			NULL		0	NULL	NULL	NULL	gw60_genetics_158_1_109_s_190	11333222	We isolated a single complementing plasmid, and further subcloning and complementation indicated that a plasmid containing only the full-length  SAE2/ COM1 ORF (YGL175C) was sufficient for full complementation of the sporulation, MMS sensitivity, and DSB-induced mutator phenotypes (data not shown).	gene_phenotype
68862	2	333140	5	NULL	NULL	0	NULL	plasmid	CellComponent		contains		only			YGL175C	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_genetics_158_1_109_s_190	11333222	We isolated a single complementing plasmid, and further subcloning and complementation indicated that a plasmid containing only the full-length  SAE2/ COM1 ORF (YGL175C) was sufficient for full complementation of the sporulation, MMS sensitivity, and DSB-induced mutator phenotypes (data not shown).	gene_phenotype
68863	3	333140	5	NULL	NULL	0	NULL	statement 2	CellComponent		is sufficient for					sporulation	Process	full complement of			NULL		0	NULL	NULL	NULL	gw60_genetics_158_1_109_s_190	11333222	We isolated a single complementing plasmid, and further subcloning and complementation indicated that a plasmid containing only the full-length  SAE2/ COM1 ORF (YGL175C) was sufficient for full complementation of the sporulation, MMS sensitivity, and DSB-induced mutator phenotypes (data not shown).	gene_phenotype
68864	4	333140	5	NULL	NULL	0	NULL	statement 2	CellComponent		is sufficient for					MMS sensitivity	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_158_1_109_s_190	11333222	We isolated a single complementing plasmid, and further subcloning and complementation indicated that a plasmid containing only the full-length  SAE2/ COM1 ORF (YGL175C) was sufficient for full complementation of the sporulation, MMS sensitivity, and DSB-induced mutator phenotypes (data not shown).	gene_phenotype
68865	5	333140	5	NULL	NULL	NULL	NULL	mutator phenotypes			is induced by					DSB	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_genetics_158_1_109_s_190	11333222	We isolated a single complementing plasmid, and further subcloning and complementation indicated that a plasmid containing only the full-length  SAE2/ COM1 ORF (YGL175C) was sufficient for full complementation of the sporulation, MMS sensitivity, and DSB-induced mutator phenotypes (data not shown).	gene_phenotype
68866	6	333140	5	NULL	NULL	0	NULL	statement 2	CellComponent		is sufficient for					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_158_1_109_s_190	11333222	We isolated a single complementing plasmid, and further subcloning and complementation indicated that a plasmid containing only the full-length  SAE2/ COM1 ORF (YGL175C) was sufficient for full complementation of the sporulation, MMS sensitivity, and DSB-induced mutator phenotypes (data not shown).	gene_phenotype
68867	1	333141	5	NULL	NULL	0	NULL	suppressors of snf1 pcl8 pcl10	GP		affects		potentially			autophagy	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_17_5742_s_276	11486014	We also tested whether some of the other genes identified as high-copy-number suppressors of  snf1 pcl8 pcl10 affected autophagy by making deletions of  RCK2 and  YGR161C in the TN125 background.	gene_phenotype
68868	1	333142	5	NULL	NULL	0	NULL	RCK2 gene	GP	deletion of	does not affect					autophagy	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_17_5742_s_331	11486014	Note that  SNF1 may exert yet other controls over the maintenance of glycogen stores, since deletion of two of the genes identified in the genetic screen,  RCK2 and  YGR161C, does not affect autophagy.	gene_phenotype
68869	2	333142	5	NULL	NULL	0	NULL	YGR161C 	NucleicAcid		does not affect					autophagy	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_17_5742_s_331	11486014	Note that  SNF1 may exert yet other controls over the maintenance of glycogen stores, since deletion of two of the genes identified in the genetic screen,  RCK2 and  YGR161C, does not affect autophagy.	gene_phenotype
68870	3	333142	5	NULL	NULL	0	NULL	SNF1	GP		exerts		may			glycogen	Chemical	controls over;;maintenance of;;stores of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_17_5742_s_331	11486014	Note that  SNF1 may exert yet other controls over the maintenance of glycogen stores, since deletion of two of the genes identified in the genetic screen,  RCK2 and  YGR161C, does not affect autophagy.	gene_phenotype
68872	1	333143	5	NULL	NULL	0	NULL	polypeptides	GP		fold into					three-dimensional conformations	GP				NULL	within the ER	0	NULL	NULL	NULL	gw60_embo_17_12_3251_s_12	9628862	Commonly coupled with the translocation process, the polypeptides fold into their three-dimensional conformations within the ER where they may assemble with other proteins into oligomeric complexes.	gene_phenotype
68873	2	333143	5	NULL	NULL	NULL	NULL	statement 1	Process		leads to					oligomeric complexes	GP	formation of			NULL	within the ER	NULL	NULL	NULL	NULL	gw60_embo_17_12_3251_s_12	9628862	Commonly coupled with the translocation process, the polypeptides fold into their three-dimensional conformations within the ER where they may assemble with other proteins into oligomeric complexes.	gene_phenotype
68874	3	333143	5	NULL	NULL	0	NULL	statement 1	Process		is coupled with					translocation	Process				NULL		0	NULL	NULL	NULL	gw60_embo_17_12_3251_s_12	9628862	Commonly coupled with the translocation process, the polypeptides fold into their three-dimensional conformations within the ER where they may assemble with other proteins into oligomeric complexes.	gene_phenotype
68875	1	333145	5	NULL	NULL	0	NULL	YMR216C locus	NucleicAcid		corresponds to					SKY1 gene	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_3_659_s_88	11854447	The YMR216C locus corresponds to the  SKY1 (SR-protein-specific kinase from budding yeast) gene, which encodes a protein serine/threonine kinase with structural and functional homology to the human SR-protein-specific kinases (SRPKs).	gene_phenotype
68876	2	333145	5	NULL	NULL	0	NULL	SKY1	GP		is					SR-protein-specific kinase from budding yeast	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_3_659_s_88	11854447	The YMR216C locus corresponds to the  SKY1 (SR-protein-specific kinase from budding yeast) gene, which encodes a protein serine/threonine kinase with structural and functional homology to the human SR-protein-specific kinases (SRPKs).	gene_phenotype
68877	3	333145	5	NULL	NULL	0	NULL	SKY1 gene	GP		encodes					protein serine/threonine kinase	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_3_659_s_88	11854447	The YMR216C locus corresponds to the  SKY1 (SR-protein-specific kinase from budding yeast) gene, which encodes a protein serine/threonine kinase with structural and functional homology to the human SR-protein-specific kinases (SRPKs).	gene_phenotype
68878	4	333145	5	NULL	NULL	0	NULL	protein serine/threonine kinase	GP		is homologous to		structurally;;funtionally			SRPKs	GP	human			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_3_659_s_88	11854447	The YMR216C locus corresponds to the  SKY1 (SR-protein-specific kinase from budding yeast) gene, which encodes a protein serine/threonine kinase with structural and functional homology to the human SR-protein-specific kinases (SRPKs).	gene_phenotype
68879	5	333145	5	NULL	NULL	0	NULL	SRPKs	GP		is					SR-protein-specific kinases	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_3_659_s_88	11854447	The YMR216C locus corresponds to the  SKY1 (SR-protein-specific kinase from budding yeast) gene, which encodes a protein serine/threonine kinase with structural and functional homology to the human SR-protein-specific kinases (SRPKs).	gene_phenotype
68880	1	333148	5	NULL	NULL	0	NULL	Dus2	GP		is encoded by					ORF YNR015w	NucleicAcid				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_rna_8_3_12003496_s_6	12003496	We show that one of these proteins, Dus2,  encoded by ORF YNR015w, has activity with two other substrates: yeast  pre-tRNA(Tyr) and pre-tRNA(Leu).	gene_phenotype
68881	2	333148	5	NULL	NULL	0	NULL	Dus2	GP		has activity with					pre-tRNA(Tyr)	NucleicAcid	yeast			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_rna_8_3_12003496_s_6	12003496	We show that one of these proteins, Dus2,  encoded by ORF YNR015w, has activity with two other substrates: yeast  pre-tRNA(Tyr) and pre-tRNA(Leu).	gene_phenotype
68882	3	333148	5	NULL	NULL	0	NULL	Dus2	GP		has activity with					pre-tRNA(Leu)	NucleicAcid	yeast			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_rna_8_3_12003496_s_6	12003496	We show that one of these proteins, Dus2,  encoded by ORF YNR015w, has activity with two other substrates: yeast  pre-tRNA(Tyr) and pre-tRNA(Leu).	gene_phenotype
68883	1	333151	5	NULL	NULL	0	NULL	PRL1	GP		is similar to					family of WD proteins	GP				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_19_3059_s_159	9765207	In the database, PRL1 identified a family of WD proteins with unknown function: PRL2 from  Arabidopsis shared 83%, PRL1 from fission yeast 69%, YPL151c from budding yeast 63% (Purnelle et al. 1996  ), and hypothetical gene product D1054.15 from  Caenorhabditis 62% sequence identity with PRL1.	gene_phenotype
68884	2	333151	5	NULL	NULL	0	NULL	PRL2	GP	Arabidopsis	is similar to					PRL1	GP				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_19_3059_s_159	9765207	In the database, PRL1 identified a family of WD proteins with unknown function: PRL2 from  Arabidopsis shared 83%, PRL1 from fission yeast 69%, YPL151c from budding yeast 63% (Purnelle et al. 1996  ), and hypothetical gene product D1054.15 from  Caenorhabditis 62% sequence identity with PRL1.	gene_phenotype
68885	3	333151	5	NULL	NULL	0	NULL	PRL1	GP	fission yeast	is similar to					PRL1	GP				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_19_3059_s_159	9765207	In the database, PRL1 identified a family of WD proteins with unknown function: PRL2 from  Arabidopsis shared 83%, PRL1 from fission yeast 69%, YPL151c from budding yeast 63% (Purnelle et al. 1996  ), and hypothetical gene product D1054.15 from  Caenorhabditis 62% sequence identity with PRL1.	gene_phenotype
68886	4	333151	5	NULL	NULL	0	NULL	YPL151c	NucleicAcid	budding yeast	is similar to					PRL1	GP				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_19_3059_s_159	9765207	In the database, PRL1 identified a family of WD proteins with unknown function: PRL2 from  Arabidopsis shared 83%, PRL1 from fission yeast 69%, YPL151c from budding yeast 63% (Purnelle et al. 1996  ), and hypothetical gene product D1054.15 from  Caenorhabditis 62% sequence identity with PRL1.	gene_phenotype
68887	5	333151	5	NULL	NULL	0	NULL	D1054.15	GP	hypothetical gene product;;Caenorhabditis	is similar to					PRL1	GP				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_19_3059_s_159	9765207	In the database, PRL1 identified a family of WD proteins with unknown function: PRL2 from  Arabidopsis shared 83%, PRL1 from fission yeast 69%, YPL151c from budding yeast 63% (Purnelle et al. 1996  ), and hypothetical gene product D1054.15 from  Caenorhabditis 62% sequence identity with PRL1.	gene_phenotype
68888	1	333152	5	NULL	NULL	0	NULL	YBL009W	NucleicAcid		is induced during		significantly			sporulation	Process				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_4_472_s_365	15681610	The second homolog,  YBL009W, is significantly induced during sporulation (Chu et al. 1998 ).	gene_phenotype
68889	1	333153	5	NULL	NULL	0	NULL	Alk1p	GP		function during					mitosis	Process				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_4_472_s_366	15681610	The data suggest that Alk1p and Ybl009wp function during mitosis and meiosis, respectively (Higgins 2003 ).	gene_phenotype
68890	2	333153	5	NULL	NULL	0	NULL	Ybl009wp	NucleicAcid		function during					meiosis	Process				NULL		0	NULL	NULL	NULL	gw70_genesdev_19_4_472_s_366	15681610	The data suggest that Alk1p and Ybl009wp function during mitosis and meiosis, respectively (Higgins 2003 ).	gene_phenotype
68891	1	333154	5	NULL	NULL	0	NULL	KRR1T gene	GP		is essential for					Saccharomyces cerevisiae	Cell	viability of			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_5_1409_s_429	11359931	A novel cross-phylum family of proteins comprises a  KRR1T (YCL059c) gene which is essential for viability of  Saccharomyces cerevisiae cells.	gene_phenotype
68892	2	333154	5	NULL	NULL	0	NULL	YCL059c	NucleicAcid		is the locus name of					KRR1T	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_5_1409_s_429	11359931	A novel cross-phylum family of proteins comprises a  KRR1T (YCL059c) gene which is essential for viability of  Saccharomyces cerevisiae cells.	gene_phenotype
68893	1	333156	5	NULL	NULL	0	NULL	KRR1T	GP	Saccharomyces cerevisiae	is essential for					cell viability	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_acta-biochim-pol_47_4_11996121_s_2	11996121	The newly discovered Saccharomyces cerevisiae gene KRR1 (YCL059c) encodes  a protein essential for cell viability.	gene_phenotype
68894	2	333156	5	NULL	NULL	0	NULL	YCL059c	NucleicAcid		is the locus name of					KRR1	GP				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_acta-biochim-pol_47_4_11996121_s_2	11996121	The newly discovered Saccharomyces cerevisiae gene KRR1 (YCL059c) encodes  a protein essential for cell viability.	gene_phenotype
68895	1	333159	5	NULL	NULL	0	NULL	YCR052w	NucleicAcid		is essential for					mitotic growth	Process				NULL		0	NULL	NULL	NULL	gw60_cell_87_7_1249_s_33	8980231	All  inviable spores germinated and divided three or four times, showing that  YCR052w is  essential for mitotic growth (  Figure 1).	gene_phenotype
68951	1	333161	5	NULL	NULL	NULL	NULL	YDL020C	NucleicAcid		is associated with		may be;;loosely			proteasome	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_1_262_s_194	10618406	Both YDL020C and YDR069C may be loosely associated with the proteasome ( 23-25), but the SVM does not classify them as belonging to the proteasome because they are regulated differently from the rest of the proteasome during sporulation.	gene_phenotype
68952	2	333161	5	NULL	NULL	NULL	NULL	YDR069C	NucleicAcid		is associated with		may be;;loosely			proteasome	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_1_262_s_194	10618406	Both YDL020C and YDR069C may be loosely associated with the proteasome ( 23-25), but the SVM does not classify them as belonging to the proteasome because they are regulated differently from the rest of the proteasome during sporulation.	gene_phenotype
68953	1	333163	5	NULL	NULL	0	NULL	YFL049W	NucleicAcid		is a type of					transcriptional regulator	GP				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_34_3_955_s_9	16464826	Based on their transcriptional activity, localization and interaction patterns, at least six previously uncharacterized proteins are suggested to be bona fide transcriptional regulators (namely YFL049W, YJR070C, YDR520C, YGL066W/Sgf73, YKR064W and YCR082W/Ahc2).	gene_phenotype
68954	2	333163	5	NULL	NULL	0	NULL	YJR070C	NucleicAcid		is a type of					transcriptional regulator	GP				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_34_3_955_s_9	16464826	Based on their transcriptional activity, localization and interaction patterns, at least six previously uncharacterized proteins are suggested to be bona fide transcriptional regulators (namely YFL049W, YJR070C, YDR520C, YGL066W/Sgf73, YKR064W and YCR082W/Ahc2).	gene_phenotype
68955	3	333163	5	NULL	NULL	0	NULL	YDR520C	NucleicAcid		is a type of					transcriptional regulator	GP				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_34_3_955_s_9	16464826	Based on their transcriptional activity, localization and interaction patterns, at least six previously uncharacterized proteins are suggested to be bona fide transcriptional regulators (namely YFL049W, YJR070C, YDR520C, YGL066W/Sgf73, YKR064W and YCR082W/Ahc2).	gene_phenotype
68956	4	333163	5	NULL	NULL	0	NULL	Sgf73	GP		is a type of					transcriptional regulator	GP				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_34_3_955_s_9	16464826	Based on their transcriptional activity, localization and interaction patterns, at least six previously uncharacterized proteins are suggested to be bona fide transcriptional regulators (namely YFL049W, YJR070C, YDR520C, YGL066W/Sgf73, YKR064W and YCR082W/Ahc2).	gene_phenotype
68957	5	333163	5	NULL	NULL	0	NULL	YKR064W	NucleicAcid		is a type of					transcriptional regulator	GP				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_34_3_955_s_9	16464826	Based on their transcriptional activity, localization and interaction patterns, at least six previously uncharacterized proteins are suggested to be bona fide transcriptional regulators (namely YFL049W, YJR070C, YDR520C, YGL066W/Sgf73, YKR064W and YCR082W/Ahc2).	gene_phenotype
68958	6	333163	5	NULL	NULL	0	NULL	Ahc2	GP		is a type of					transcriptional regulator	GP				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_34_3_955_s_9	16464826	Based on their transcriptional activity, localization and interaction patterns, at least six previously uncharacterized proteins are suggested to be bona fide transcriptional regulators (namely YFL049W, YJR070C, YDR520C, YGL066W/Sgf73, YKR064W and YCR082W/Ahc2).	gene_phenotype
68959	7	333163	5	NULL	NULL	0	NULL	YGL066W	NucleicAcid		is the locus name of					Sgf73	GP				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_34_3_955_s_9	16464826	Based on their transcriptional activity, localization and interaction patterns, at least six previously uncharacterized proteins are suggested to be bona fide transcriptional regulators (namely YFL049W, YJR070C, YDR520C, YGL066W/Sgf73, YKR064W and YCR082W/Ahc2).	gene_phenotype
68960	8	333163	5	NULL	NULL	0	NULL	YCR082W	NucleicAcid		is the locus name of					Ahc2	GP				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_34_3_955_s_9	16464826	Based on their transcriptional activity, localization and interaction patterns, at least six previously uncharacterized proteins are suggested to be bona fide transcriptional regulators (namely YFL049W, YJR070C, YDR520C, YGL066W/Sgf73, YKR064W and YCR082W/Ahc2).	gene_phenotype
68961	1	333168	5	NULL	NULL	0	NULL	YJL125c	NucleicAcid	Saccharomyces cerevisiae	is essential for					vegetative growth	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_20_7784_s_461	11003673	Disruption and basic functional analysis of five chromosome X novel ORFs of Saccharomyces cerevisiae reveals YJL125c as an essential gene for vegetative growth.	gene_phenotype
68962	1	333174	5	NULL	NULL	0	NULL	YLR126C	NucleicAcid		encodes					COG0518.1, GuaA			glutamine amidotransferase domain		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_6_4450_s_229	14534306	YLR126C encodes a protein with a glutamine amidotransferase domain (COG0518.1, GuaA), which is present in multiple proteins involved in nucleotide transport or metabolism as well as anthranilate synthases.	gene_phenotype
68963	2	333174	5	NULL	NULL	0	NULL	proteins	GP		is involved in			glutamine amidotransferase domain		nucleotide transport	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_6_4450_s_229	14534306	YLR126C encodes a protein with a glutamine amidotransferase domain (COG0518.1, GuaA), which is present in multiple proteins involved in nucleotide transport or metabolism as well as anthranilate synthases.	gene_phenotype
68964	3	333174	5	NULL	NULL	0	NULL	proteins	GP		is involved in			glutamine amidotransferase domain		metabolism	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_6_4450_s_229	14534306	YLR126C encodes a protein with a glutamine amidotransferase domain (COG0518.1, GuaA), which is present in multiple proteins involved in nucleotide transport or metabolism as well as anthranilate synthases.	gene_phenotype
68965	4	333174	5	NULL	NULL	0	NULL	YLR126C	NucleicAcid		encodes					anthranilate synthases	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_6_4450_s_229	14534306	YLR126C encodes a protein with a glutamine amidotransferase domain (COG0518.1, GuaA), which is present in multiple proteins involved in nucleotide transport or metabolism as well as anthranilate synthases.	gene_phenotype
68966	1	333175	5	NULL	NULL	0	NULL	YPR128C	NucleicAcid		is a member of					ATP/ADP carrier family of solute transporters	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_96_6_2937_s_108	10077615	The search for candidate PMPs was also successful, leading to the identification of YPR128C, an uncharacterized member of the ATP/ADP carrier family of solute transporters, and YOL044W, an orphan protein.	gene_phenotype
68967	2	333175	5	NULL	NULL	0	NULL	YOL044W	NucleicAcid		is a type of					orphan protein	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_96_6_2937_s_108	10077615	The search for candidate PMPs was also successful, leading to the identification of YPR128C, an uncharacterized member of the ATP/ADP carrier family of solute transporters, and YOL044W, an orphan protein.	gene_phenotype
68968	1	333178	5	NULL	NULL	0	NULL	YKR096w	NucleicAcid		is dispensable for					cell viability	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_103_25_9464_s_51	16769905	This effect is consistent with results from a large-scale deletion project that found YKR096w and YOR166c dispensable for cell viability ( ).	gene_phenotype
68969	2	333178	5	NULL	NULL	0	NULL	YOR166c	NucleicAcid		is dispensable for					cell viability	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_103_25_9464_s_51	16769905	This effect is consistent with results from a large-scale deletion project that found YKR096w and YOR166c dispensable for cell viability ( ).	gene_phenotype
68970	1	333181	5	NULL	NULL	NULL	NULL	aut4	Cell		is defective in					autophagic vesicles	CellComponent	lysis of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17621_s_102	8663607	Interestingly,  aut4 and  aut6 have different autophagy defects:  aut4, like  aut5, is defective in lysis of autophagic vesicles after delivery to the vacuole; vesicles accumulate in the vacuole in the absence of PMSF.  aut6, similar to  aut1,  2,  3, and  9, is defective in accumulation of vesicles	gene_phenotype
68971	2	333181	5	NULL	NULL	0	NULL	statement 1	Process		occurs after					vacuole	CellComponent	delivery to			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_30_17621_s_102	8663607	Interestingly,  aut4 and  aut6 have different autophagy defects:  aut4, like  aut5, is defective in lysis of autophagic vesicles after delivery to the vacuole; vesicles accumulate in the vacuole in the absence of PMSF.  aut6, similar to  aut1,  2,  3, and  9, is defective in accumulation of vesicles	gene_phenotype
68972	3	333181	5	NULL	NULL	NULL	NULL	aut5	Cell		is defective in					autophagic vesicles	CellComponent	lysis of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_30_17621_s_102	8663607	Interestingly,  aut4 and  aut6 have different autophagy defects:  aut4, like  aut5, is defective in lysis of autophagic vesicles after delivery to the vacuole; vesicles accumulate in the vacuole in the absence of PMSF.  aut6, similar to  aut1,  2,  3, and  9, is defective in accumulation of vesicles	gene_phenotype
68973	4	333181	5	NULL	NULL	0	NULL	vesicles	CellComponent		accumulates in					vacuole	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_30_17621_s_102	8663607	Interestingly,  aut4 and  aut6 have different autophagy defects:  aut4, like  aut5, is defective in lysis of autophagic vesicles after delivery to the vacuole; vesicles accumulate in the vacuole in the absence of PMSF.  aut6, similar to  aut1,  2,  3, and  9, is defective in accumulation of vesicles	gene_phenotype
68974	5	333181	5	NULL	NULL	0	NULL	statement 4	Process		in the absence of					PMSF	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_30_17621_s_102	8663607	Interestingly,  aut4 and  aut6 have different autophagy defects:  aut4, like  aut5, is defective in lysis of autophagic vesicles after delivery to the vacuole; vesicles accumulate in the vacuole in the absence of PMSF.  aut6, similar to  aut1,  2,  3, and  9, is defective in accumulation of vesicles	gene_phenotype
68975	6	333181	5	NULL	NULL	0	NULL	aut6	Cell		is defective in					vesicle	CellComponent	accumulation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_30_17621_s_102	8663607	Interestingly,  aut4 and  aut6 have different autophagy defects:  aut4, like  aut5, is defective in lysis of autophagic vesicles after delivery to the vacuole; vesicles accumulate in the vacuole in the absence of PMSF.  aut6, similar to  aut1,  2,  3, and  9, is defective in accumulation of vesicles	gene_phenotype
68976	7	333181	5	NULL	NULL	0	NULL	aut1	Cell		is defective in					vesicle	CellComponent	accumulation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_30_17621_s_102	8663607	Interestingly,  aut4 and  aut6 have different autophagy defects:  aut4, like  aut5, is defective in lysis of autophagic vesicles after delivery to the vacuole; vesicles accumulate in the vacuole in the absence of PMSF.  aut6, similar to  aut1,  2,  3, and  9, is defective in accumulation of vesicles	gene_phenotype
68977	8	333181	5	NULL	NULL	0	NULL	aut2	Cell		is defective in					vesicle	CellComponent	accumulation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_30_17621_s_102	8663607	Interestingly,  aut4 and  aut6 have different autophagy defects:  aut4, like  aut5, is defective in lysis of autophagic vesicles after delivery to the vacuole; vesicles accumulate in the vacuole in the absence of PMSF.  aut6, similar to  aut1,  2,  3, and  9, is defective in accumulation of vesicles	gene_phenotype
68978	9	333181	5	NULL	NULL	0	NULL	aut3	Cell		is defective in					vesicle	CellComponent	accumulation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_30_17621_s_102	8663607	Interestingly,  aut4 and  aut6 have different autophagy defects:  aut4, like  aut5, is defective in lysis of autophagic vesicles after delivery to the vacuole; vesicles accumulate in the vacuole in the absence of PMSF.  aut6, similar to  aut1,  2,  3, and  9, is defective in accumulation of vesicles	gene_phenotype
68979	10	333181	5	NULL	NULL	0	NULL	aut9	Cell		is defective in					vesicle	CellComponent	accumulation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_30_17621_s_102	8663607	Interestingly,  aut4 and  aut6 have different autophagy defects:  aut4, like  aut5, is defective in lysis of autophagic vesicles after delivery to the vacuole; vesicles accumulate in the vacuole in the absence of PMSF.  aut6, similar to  aut1,  2,  3, and  9, is defective in accumulation of vesicles	gene_phenotype
68980	1	333182	5	NULL	NULL	NULL	NULL	cvt3	Process		is defective in					API	GP	maturation of			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_21_6005_s_252	10545112	This corroborates previous findings, in which the API maturation defects of  cvt3 and  cvt9 were found to be bypassed by the autophagy pathway, and two mutants defective in autophagy,  aut4 and  aut6, were found to process API normally (Harding  et al., 1996  ).	gene_phenotype
68981	2	333182	5	NULL	NULL	0	NULL	cvt9	Process		is defective in					API	GP	maturation of			NULL		0	NULL	NULL	NULL	gw60_embo_18_21_6005_s_252	10545112	This corroborates previous findings, in which the API maturation defects of  cvt3 and  cvt9 were found to be bypassed by the autophagy pathway, and two mutants defective in autophagy,  aut4 and  aut6, were found to process API normally (Harding  et al., 1996  ).	gene_phenotype
68982	3	333182	5	NULL	NULL	0	NULL	statement 1	Process		is bypassed by					autophagy pathway	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_21_6005_s_252	10545112	This corroborates previous findings, in which the API maturation defects of  cvt3 and  cvt9 were found to be bypassed by the autophagy pathway, and two mutants defective in autophagy,  aut4 and  aut6, were found to process API normally (Harding  et al., 1996  ).	gene_phenotype
68983	4	333182	5	NULL	NULL	0	NULL	statement 2	Process		is bypassed by					autophagy pathway	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_21_6005_s_252	10545112	This corroborates previous findings, in which the API maturation defects of  cvt3 and  cvt9 were found to be bypassed by the autophagy pathway, and two mutants defective in autophagy,  aut4 and  aut6, were found to process API normally (Harding  et al., 1996  ).	gene_phenotype
68984	5	333182	5	NULL	NULL	0	NULL	aut4	Cell		is defective in					autophagy	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_21_6005_s_252	10545112	This corroborates previous findings, in which the API maturation defects of  cvt3 and  cvt9 were found to be bypassed by the autophagy pathway, and two mutants defective in autophagy,  aut4 and  aut6, were found to process API normally (Harding  et al., 1996  ).	gene_phenotype
68985	6	333182	5	NULL	NULL	0	NULL	aut6	Cell		is defective in					autophagy	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_21_6005_s_252	10545112	This corroborates previous findings, in which the API maturation defects of  cvt3 and  cvt9 were found to be bypassed by the autophagy pathway, and two mutants defective in autophagy,  aut4 and  aut6, were found to process API normally (Harding  et al., 1996  ).	gene_phenotype
68986	7	333182	5	NULL	NULL	0	NULL	aut4	Cell		process		normally			API	GP				NULL		0	NULL	NULL	NULL	gw60_embo_18_21_6005_s_252	10545112	This corroborates previous findings, in which the API maturation defects of  cvt3 and  cvt9 were found to be bypassed by the autophagy pathway, and two mutants defective in autophagy,  aut4 and  aut6, were found to process API normally (Harding  et al., 1996  ).	gene_phenotype
68987	8	333182	5	NULL	NULL	0	NULL	aut6	Cell		process		normally			API	GP				NULL		0	NULL	NULL	NULL	gw60_embo_18_21_6005_s_252	10545112	This corroborates previous findings, in which the API maturation defects of  cvt3 and  cvt9 were found to be bypassed by the autophagy pathway, and two mutants defective in autophagy,  aut4 and  aut6, were found to process API normally (Harding  et al., 1996  ).	gene_phenotype
68988	1	333183	5	NULL	NULL	0	NULL	DAL5	GP		is a synonym of					allantoate permease	GP				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_21_2_113_s_157	9348664	The allantoate permease YJR152w ( DAL5) has given its name to the family, the other members of which might transport other  weak acids and include the proteins YAl067c ( GEO1) and YCR028c ( FEN2), which are both involved in some kind of resistance.	gene_phenotype
68989	2	333183	5	NULL	NULL	0	NULL	YJR152w	NucleicAcid		is the locus name of					DAL5	GP				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_21_2_113_s_157	9348664	The allantoate permease YJR152w ( DAL5) has given its name to the family, the other members of which might transport other  weak acids and include the proteins YAl067c ( GEO1) and YCR028c ( FEN2), which are both involved in some kind of resistance.	gene_phenotype
68990	3	333183	5	NULL	NULL	0	NULL	DAL5	GP		transport		might			acids	Chemical	weak			NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_21_2_113_s_157	9348664	The allantoate permease YJR152w ( DAL5) has given its name to the family, the other members of which might transport other  weak acids and include the proteins YAl067c ( GEO1) and YCR028c ( FEN2), which are both involved in some kind of resistance.	gene_phenotype
68991	4	333183	5	NULL	NULL	0	NULL	GEO1	GP		is involved in					resistance	Process				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_21_2_113_s_157	9348664	The allantoate permease YJR152w ( DAL5) has given its name to the family, the other members of which might transport other  weak acids and include the proteins YAl067c ( GEO1) and YCR028c ( FEN2), which are both involved in some kind of resistance.	gene_phenotype
68992	5	333183	5	NULL	NULL	0	NULL	FEN2	GP		is involved in					resistance	Process				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_21_2_113_s_157	9348664	The allantoate permease YJR152w ( DAL5) has given its name to the family, the other members of which might transport other  weak acids and include the proteins YAl067c ( GEO1) and YCR028c ( FEN2), which are both involved in some kind of resistance.	gene_phenotype
68993	6	333183	5	NULL	NULL	0	NULL	YAl067c	NucleicAcid		is the locus name of					GEO1	GP				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_21_2_113_s_157	9348664	The allantoate permease YJR152w ( DAL5) has given its name to the family, the other members of which might transport other  weak acids and include the proteins YAl067c ( GEO1) and YCR028c ( FEN2), which are both involved in some kind of resistance.	gene_phenotype
68994	7	333183	5	NULL	NULL	0	NULL	YCR028c	NucleicAcid		is the locus name of					FEN2	GP				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_21_2_113_s_157	9348664	The allantoate permease YJR152w ( DAL5) has given its name to the family, the other members of which might transport other  weak acids and include the proteins YAl067c ( GEO1) and YCR028c ( FEN2), which are both involved in some kind of resistance.	gene_phenotype
68995	1	333184	5	NULL	NULL	0	NULL	UGA2	GP		is a synonym of					SSADH	GP	yeast			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_42_41552_s_81	12882961	This mutant had only approximately 10% of the SSADH activity of the wild-type strain when grown on GABA as the sole nitrogen source (2.3 and 24.8 mumol/h/mg protein, respectively) and was found to overlap the YBR006W locus (data not shown), confirming that UGA2/YBR006w is the yeast SSADH ( ).	gene_phenotype
68996	2	333184	5	NULL	NULL	0	NULL	YBR006w	NucleicAcid		is the locus name of					UGA2	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_42_41552_s_81	12882961	This mutant had only approximately 10% of the SSADH activity of the wild-type strain when grown on GABA as the sole nitrogen source (2.3 and 24.8 mumol/h/mg protein, respectively) and was found to overlap the YBR006W locus (data not shown), confirming that UGA2/YBR006w is the yeast SSADH ( ).	gene_phenotype
68997	1	333185	5	NULL	NULL	0	NULL	YIH1	GP		is					yeast impact homolog 1	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20243_s_52	10801780	As an approach to revealing the function of this protein family, we analyzed its budding yeast homolog YCR059C, or  yeast  impact  homolog 1 (YIH1), and identified GCN1 as its potential binding partner through a two-hybrid screening.	gene_phenotype
68998	2	333185	5	NULL	NULL	0	NULL	YIH1	GP		bind		potentially			GCN1	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20243_s_52	10801780	As an approach to revealing the function of this protein family, we analyzed its budding yeast homolog YCR059C, or  yeast  impact  homolog 1 (YIH1), and identified GCN1 as its potential binding partner through a two-hybrid screening.	gene_phenotype
68999	3	333185	5	NULL	NULL	0	NULL	YCR059C	NucleicAcid	budding yeast	bind		potentially			GCN1	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20243_s_52	10801780	As an approach to revealing the function of this protein family, we analyzed its budding yeast homolog YCR059C, or  yeast  impact  homolog 1 (YIH1), and identified GCN1 as its potential binding partner through a two-hybrid screening.	gene_phenotype
69000	1	333187	5	NULL	NULL	0	NULL	Ydr532c protein	GP		is a component of					SPB	CellComponent				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_12_5255_s_250	15371542	The 44-kDa Ydr532c protein has been identified as a component of the SPB and very recently as a new component of the budding yeast kinetochore (Giaever  et al., 2002 ;	gene_phenotype
69001	2	333187	5	NULL	NULL	0	NULL	Ydr532c protein	GP		is a component of					kinetochore	CellComponent	budding yeast			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_12_5255_s_250	15371542	The 44-kDa Ydr532c protein has been identified as a component of the SPB and very recently as a new component of the budding yeast kinetochore (Giaever  et al., 2002 ;	gene_phenotype
69002	1	333188	5	NULL	NULL	0	NULL	YER004W gene	GP		is a homolog of					Tip30 protein	GP	human			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_10_2987_s_304	11598186	Interestingly, the gene  YER004W has homology to the human protein Tip30, a tumor suppressor that mediates apoptosis (Shtivelman, 1997  ; Xiao  et al., 1998  , 2000  ), but its function in yeast remains to be discovered.	gene_phenotype
69003	2	333188	5	NULL	NULL	0	NULL	Tip30 protein	GP	human	is a type of					tumor suppressor	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_10_2987_s_304	11598186	Interestingly, the gene  YER004W has homology to the human protein Tip30, a tumor suppressor that mediates apoptosis (Shtivelman, 1997  ; Xiao  et al., 1998  , 2000  ), but its function in yeast remains to be discovered.	gene_phenotype
69004	3	333188	5	NULL	NULL	0	NULL	Tip30 protein	GP	human	mediates					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_10_2987_s_304	11598186	Interestingly, the gene  YER004W has homology to the human protein Tip30, a tumor suppressor that mediates apoptosis (Shtivelman, 1997  ; Xiao  et al., 1998  , 2000  ), but its function in yeast remains to be discovered.	gene_phenotype
69005	1	333189	5	NULL	NULL	0	NULL	Pth2	GP		is involved in					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_3_1436_s_266	16407407	We also identified homologues of mammalian proteins involved in apoptosis, such as Pth2 (a homologue of human Bit1; Jan  et al., 2004 ), Ndi1 (a homologue of AMID; Wu  et al., 2002 ), and Yer004w, which is homologous to mammalian HTATIP2, a protein acting in tumor suppression and apoptosis (Hodges  et al., 2002 ).	gene_phenotype
69006	2	333189	5	NULL	NULL	0	NULL	Pth2	GP		is a homolog of					Bit1	GP	human			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_3_1436_s_266	16407407	We also identified homologues of mammalian proteins involved in apoptosis, such as Pth2 (a homologue of human Bit1; Jan  et al., 2004 ), Ndi1 (a homologue of AMID; Wu  et al., 2002 ), and Yer004w, which is homologous to mammalian HTATIP2, a protein acting in tumor suppression and apoptosis (Hodges  et al., 2002 ).	gene_phenotype
69007	3	333189	5	NULL	NULL	0	NULL	Ndi1	GP		is involved in					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_3_1436_s_266	16407407	We also identified homologues of mammalian proteins involved in apoptosis, such as Pth2 (a homologue of human Bit1; Jan  et al., 2004 ), Ndi1 (a homologue of AMID; Wu  et al., 2002 ), and Yer004w, which is homologous to mammalian HTATIP2, a protein acting in tumor suppression and apoptosis (Hodges  et al., 2002 ).	gene_phenotype
69008	4	333189	5	NULL	NULL	0	NULL	Ndi1	GP		is a homolog of					AMID	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_3_1436_s_266	16407407	We also identified homologues of mammalian proteins involved in apoptosis, such as Pth2 (a homologue of human Bit1; Jan  et al., 2004 ), Ndi1 (a homologue of AMID; Wu  et al., 2002 ), and Yer004w, which is homologous to mammalian HTATIP2, a protein acting in tumor suppression and apoptosis (Hodges  et al., 2002 ).	gene_phenotype
69009	5	333189	5	NULL	NULL	0	NULL	Yer004w	GP		is a homolog of					HTATIP2	GP	mammalian			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_3_1436_s_266	16407407	We also identified homologues of mammalian proteins involved in apoptosis, such as Pth2 (a homologue of human Bit1; Jan  et al., 2004 ), Ndi1 (a homologue of AMID; Wu  et al., 2002 ), and Yer004w, which is homologous to mammalian HTATIP2, a protein acting in tumor suppression and apoptosis (Hodges  et al., 2002 ).	gene_phenotype
69010	6	333189	5	NULL	NULL	NULL	NULL	HTATIP2 protein	GP	mammalian	plays a role in					tuomr supression	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_17_3_1436_s_266	16407407	We also identified homologues of mammalian proteins involved in apoptosis, such as Pth2 (a homologue of human Bit1; Jan  et al., 2004 ), Ndi1 (a homologue of AMID; Wu  et al., 2002 ), and Yer004w, which is homologous to mammalian HTATIP2, a protein acting in tumor suppression and apoptosis (Hodges  et al., 2002 ).	gene_phenotype
69011	7	333189	5	NULL	NULL	0	NULL	HTATIP2 protein	GP	mammalian	plays a role in					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_3_1436_s_266	16407407	We also identified homologues of mammalian proteins involved in apoptosis, such as Pth2 (a homologue of human Bit1; Jan  et al., 2004 ), Ndi1 (a homologue of AMID; Wu  et al., 2002 ), and Yer004w, which is homologous to mammalian HTATIP2, a protein acting in tumor suppression and apoptosis (Hodges  et al., 2002 ).	gene_phenotype
69012	1	333191	5	NULL	NULL	0	NULL	Avt proteins	GP		is related to					synaptic vesicular transporters	CellComponent	Caenorhabditis elegans;;rat;;mouse			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_44_43051_s_240	12937179	Sequence analysis predicts that the three Avt proteins are related to the synaptic vesicular transporters found in  Caenorhabditis elegans, rat, and mouse; the protein encoded by  YER053C is a member of the mitochondrial carrier family.	gene_phenotype
69013	2	333191	5	NULL	NULL	0	NULL	protein encoded by YER053C	GP		is a member of					mitochondrial carrier family	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_44_43051_s_240	12937179	Sequence analysis predicts that the three Avt proteins are related to the synaptic vesicular transporters found in  Caenorhabditis elegans, rat, and mouse; the protein encoded by  YER053C is a member of the mitochondrial carrier family.	gene_phenotype
69014	1	333193	5	NULL	NULL	0	NULL	YFR022w	NucleicAcid	expression of	downregulated in					meiosis	Process				NULL		0	NULL	NULL	NULL	gw70_nature_430_6999_573_s_71	15229615	For example, YFR022w expression is downregulated in meiosis, and the locus now was  covered by cohesin extending from the neighbouring  PES4/YFR024c association site ( Supplementary Fig. S3).	gene_phenotype
69015	2	333193	5	NULL	NULL	0	NULL	YFR022w	NucleicAcid		is covered by					cohesin	GP				NULL		0	NULL	NULL	NULL	gw70_nature_430_6999_573_s_71	15229615	For example, YFR022w expression is downregulated in meiosis, and the locus now was  covered by cohesin extending from the neighbouring  PES4/YFR024c association site ( Supplementary Fig. S3).	gene_phenotype
69016	3	333193	5	NULL	NULL	0	NULL	cohesin	GP		extends from					PES4	GP	neighbouring association site of			NULL		0	NULL	NULL	NULL	gw70_nature_430_6999_573_s_71	15229615	For example, YFR022w expression is downregulated in meiosis, and the locus now was  covered by cohesin extending from the neighbouring  PES4/YFR024c association site ( Supplementary Fig. S3).	gene_phenotype
69017	4	333193	5	NULL	NULL	0	NULL	YFR024c	GP		is the locus name of					PES4	GP				NULL		0	NULL	NULL	NULL	gw70_nature_430_6999_573_s_71	15229615	For example, YFR022w expression is downregulated in meiosis, and the locus now was  covered by cohesin extending from the neighbouring  PES4/YFR024c association site ( Supplementary Fig. S3).	gene_phenotype
69018	1	333194	5	NULL	NULL	0	NULL	proteins encoded by YGL104c	NucleicAcid		is similar to					proteins encoded by YBR241c	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_21_1_85_s_356	9299703	The proteins  encoded by genes  YGL104c and  YBR241c display 47.4% identity to each other but less than 28% to the hexose transporters.	gene_phenotype
69019	2	333194	5	NULL	NULL	0	NULL	proteins encoded by YGL104c	NucleicAcid		is similar to					hexose transporters	GP				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_21_1_85_s_356	9299703	The proteins  encoded by genes  YGL104c and  YBR241c display 47.4% identity to each other but less than 28% to the hexose transporters.	gene_phenotype
69020	3	333194	5	NULL	NULL	0	NULL	statement 1	Process		lesser than					statement 2					NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_21_1_85_s_356	9299703	The proteins  encoded by genes  YGL104c and  YBR241c display 47.4% identity to each other but less than 28% to the hexose transporters.	gene_phenotype
69021	4	333194	5	NULL	NULL	0	NULL	proteins encoded by YBR241c	NucleicAcid		is similar to					hexose transporters	GP				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_21_1_85_s_356	9299703	The proteins  encoded by genes  YGL104c and  YBR241c display 47.4% identity to each other but less than 28% to the hexose transporters.	gene_phenotype
69022	5	333194	5	NULL	NULL	0	NULL	statement 1	Process		lesser than					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_21_1_85_s_356	9299703	The proteins  encoded by genes  YGL104c and  YBR241c display 47.4% identity to each other but less than 28% to the hexose transporters.	gene_phenotype
69023	1	333196	5	NULL	NULL	0	NULL	tetrads	Cell		is formed during					sporulation	Process				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_9_2646_s_141	11553705	We therefore conclude that a novel gene  ADY1 at  YHR185C is required for the formation of tetrads in sporulation.	gene_phenotype
69024	2	333196	5	NULL	NULL	NULL	NULL	ADY1 gene	GP	novel	is required for					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_9_2646_s_141	11553705	We therefore conclude that a novel gene  ADY1 at  YHR185C is required for the formation of tetrads in sporulation.	gene_phenotype
69025	3	333196	5	NULL	NULL	0	NULL	ADY1	GP		is encoded by					YHR185C	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_9_2646_s_141	11553705	We therefore conclude that a novel gene  ADY1 at  YHR185C is required for the formation of tetrads in sporulation.	gene_phenotype
69026	1	333197	5	NULL	NULL	0	NULL	ADY1 gene	GP	novel	is required for					sporulation	Process				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_9_2646_s_32	11553705	In a screen for genes required for sporulation, we identified a novel gene  ADY1 (accumulates dyads), corresponding to the open reading frame (ORF)  YHR185C.	gene_phenotype
69027	2	333197	5	NULL	NULL	0	NULL	ADY1 gene	GP		accumulates					dyads	Cell				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_9_2646_s_32	11553705	In a screen for genes required for sporulation, we identified a novel gene  ADY1 (accumulates dyads), corresponding to the open reading frame (ORF)  YHR185C.	gene_phenotype
69028	3	333197	5	NULL	NULL	0	NULL	ADY1 gene	GP		corresponds to					ORF YHR185C	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_9_2646_s_32	11553705	In a screen for genes required for sporulation, we identified a novel gene  ADY1 (accumulates dyads), corresponding to the open reading frame (ORF)  YHR185C.	gene_phenotype
69029	1	333198	5	NULL	NULL	0	NULL	ECM31	GP	deletion of	causes					pantothenic acid 	Chemical	auxotrophy of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_14_10794_s_149	11154694	Deletions in genes that have structural homology to the bacterial genes of the pantothenic acid pathway,  ECM31 and  YIL145c (see Fig.  1), caused pantothenic acid auxotrophy, but these strains did not grow on a beta-alanine supplement, indicating that these genes are downstream in the pathway (see Fig.  1).	gene_phenotype
69030	2	333198	5	NULL	NULL	0	NULL	YIL145c	GP	deletion of	causes					pantothenic acid	Chemical	auxotrophy of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_14_10794_s_149	11154694	Deletions in genes that have structural homology to the bacterial genes of the pantothenic acid pathway,  ECM31 and  YIL145c (see Fig.  1), caused pantothenic acid auxotrophy, but these strains did not grow on a beta-alanine supplement, indicating that these genes are downstream in the pathway (see Fig.  1).	gene_phenotype
69031	1	333199	5	NULL	NULL	0	NULL	ORF YKR031c	NucleicAcid	yeast	activates					PLD	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_5_2361_s_74	8576189	Thus, ORF  YKR031c seemed a likely candidate for a yeast protein having PLD  activity and was tentatively renamed  PLD1.	gene_phenotype
69032	2	333199	5	NULL	NULL	0	NULL	ORF YKR031c	NucleicAcid	yeast	is renamed as					PLD1	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_5_2361_s_74	8576189	Thus, ORF  YKR031c seemed a likely candidate for a yeast protein having PLD  activity and was tentatively renamed  PLD1.	gene_phenotype
69033	1	333201	5	NULL	NULL	0	NULL	FOW1	GP	sequence of	is similar to		cloely			YMR241w protein	GP	yeast;;sequence of			NULL		0	NULL	NULL	NULL	gw70_nature_431_7008_582_s_93	15457264	FOW1 shares close sequence similarity with a yeast protein  (YMR241w) required for tricarboxylic acid transport 19.	gene_phenotype
69034	2	333201	5	NULL	NULL	0	NULL	YMR241w protein	GP	yeast	is required for					tricarboxylic acid	Chemical	transport of			NULL		0	NULL	NULL	NULL	gw70_nature_431_7008_582_s_93	15457264	FOW1 shares close sequence similarity with a yeast protein  (YMR241w) required for tricarboxylic acid transport 19.	gene_phenotype
69035	1	333202	5	NULL	NULL	0	NULL	Mss4	GP		is required for					actin cytoskeleton	CellComponent	polarization of			NULL		0	NULL	NULL	NULL	gw70_embo_23_19_3747_s_5	15372071	Like Mss4, Slm1 and its homolog Slm2 (Ynl047c) were required for  actin cytoskeleton polarization and viability.	gene_phenotype
69036	2	333202	5	NULL	NULL	0	NULL	Mss4	GP		is required for					actin cytoskeleton	CellComponent	viability of			NULL		0	NULL	NULL	NULL	gw70_embo_23_19_3747_s_5	15372071	Like Mss4, Slm1 and its homolog Slm2 (Ynl047c) were required for  actin cytoskeleton polarization and viability.	gene_phenotype
69037	3	333202	5	NULL	NULL	0	NULL	Slm1	GP		is required for					actin cytoskeleton	CellComponent	polarization of			NULL		0	NULL	NULL	NULL	gw70_embo_23_19_3747_s_5	15372071	Like Mss4, Slm1 and its homolog Slm2 (Ynl047c) were required for  actin cytoskeleton polarization and viability.	gene_phenotype
69038	4	333202	5	NULL	NULL	0	NULL	Slm1	GP		is required for					actin cytoskeleton	CellComponent	viability of			NULL		0	NULL	NULL	NULL	gw70_embo_23_19_3747_s_5	15372071	Like Mss4, Slm1 and its homolog Slm2 (Ynl047c) were required for  actin cytoskeleton polarization and viability.	gene_phenotype
69039	5	333202	5	NULL	NULL	0	NULL	Slm2	GP		is required for					actin cytoskeleton	CellComponent	polarization of			NULL		0	NULL	NULL	NULL	gw70_embo_23_19_3747_s_5	15372071	Like Mss4, Slm1 and its homolog Slm2 (Ynl047c) were required for  actin cytoskeleton polarization and viability.	gene_phenotype
69040	6	333202	5	NULL	NULL	0	NULL	Slm2	GP		is required for					actin cytoskeleton	CellComponent	viability of			NULL		0	NULL	NULL	NULL	gw70_embo_23_19_3747_s_5	15372071	Like Mss4, Slm1 and its homolog Slm2 (Ynl047c) were required for  actin cytoskeleton polarization and viability.	gene_phenotype
69041	7	333202	5	NULL	NULL	0	NULL	Slm2	GP		is a homolog of					Slm1	GP				NULL		0	NULL	NULL	NULL	gw70_embo_23_19_3747_s_5	15372071	Like Mss4, Slm1 and its homolog Slm2 (Ynl047c) were required for  actin cytoskeleton polarization and viability.	gene_phenotype
69042	8	333202	5	NULL	NULL	0	NULL	Ynl047c	NucleicAcid		encodes for					Slm2	GP				NULL		0	NULL	NULL	NULL	gw70_embo_23_19_3747_s_5	15372071	Like Mss4, Slm1 and its homolog Slm2 (Ynl047c) were required for  actin cytoskeleton polarization and viability.	gene_phenotype
69043	1	333203	5	NULL	NULL	0	NULL	YHR194W gene	GP		is a synonym of					MDM31	GP				NULL		0	NULL	NULL	NULL	gw70_genetics_171_2_517_s_107	16020778	Both  YHR194W and  YOR147W genes were identified previously in a genome-wide screen for mutants with an altered mitochondrial morphology and were designated as  MDM31 and  MDM32, respectively ( IMMER et al.).	gene_phenotype
69044	2	333203	5	NULL	NULL	0	NULL	YOR147W gene	GP		is a synonym of					MDM32	GP				NULL		0	NULL	NULL	NULL	gw70_genetics_171_2_517_s_107	16020778	Both  YHR194W and  YOR147W genes were identified previously in a genome-wide screen for mutants with an altered mitochondrial morphology and were designated as  MDM31 and  MDM32, respectively ( IMMER et al.).	gene_phenotype
69045	3	333203	5	NULL	NULL	0	NULL	MDM31	GP		plays a role in					mitochondria	CellComponent	morphology of			NULL		0	NULL	NULL	NULL	gw70_genetics_171_2_517_s_107	16020778	Both  YHR194W and  YOR147W genes were identified previously in a genome-wide screen for mutants with an altered mitochondrial morphology and were designated as  MDM31 and  MDM32, respectively ( IMMER et al.).	gene_phenotype
69046	4	333203	5	NULL	NULL	0	NULL	MDM32	GP		plays a role in					mitochondria	CellComponent	morphology of			NULL		0	NULL	NULL	NULL	gw70_genetics_171_2_517_s_107	16020778	Both  YHR194W and  YOR147W genes were identified previously in a genome-wide screen for mutants with an altered mitochondrial morphology and were designated as  MDM31 and  MDM32, respectively ( IMMER et al.).	gene_phenotype
69047	1	333204	5	NULL	NULL	0	NULL	YPL176c	NucleicAcid		is a synonym of					yeast transferrin receptor-like	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_99_22_14183_s_101	12374868	A GFP fusion of yeast transferrin receptor-like YPL176c (YPL176-GFP) localized in a punctate pattern along the surface of the body of the cell, mostly excluded from the shmoo tip (Fig.  3 c), and also was detergent-soluble (Fig.  3g).	gene_phenotype
69048	2	333204	5	NULL	NULL	0	NULL	YPL176-GFP	GP		is a type of					GFP fusion protein					NULL		0	NULL	NULL	NULL	gw60_pnas_99_22_14183_s_101	12374868	A GFP fusion of yeast transferrin receptor-like YPL176c (YPL176-GFP) localized in a punctate pattern along the surface of the body of the cell, mostly excluded from the shmoo tip (Fig.  3 c), and also was detergent-soluble (Fig.  3g).	gene_phenotype
69049	3	333204	5	NULL	NULL	0	NULL	YPL176-GFP	GP		is localized along					cell	Cell	surface of;;body of			NULL		0	NULL	NULL	NULL	gw60_pnas_99_22_14183_s_101	12374868	A GFP fusion of yeast transferrin receptor-like YPL176c (YPL176-GFP) localized in a punctate pattern along the surface of the body of the cell, mostly excluded from the shmoo tip (Fig.  3 c), and also was detergent-soluble (Fig.  3g).	gene_phenotype
69050	4	333204	5	NULL	NULL	0	NULL	statement 3	Process		occurs in					punctate pattern	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	gw60_pnas_99_22_14183_s_101	12374868	A GFP fusion of yeast transferrin receptor-like YPL176c (YPL176-GFP) localized in a punctate pattern along the surface of the body of the cell, mostly excluded from the shmoo tip (Fig.  3 c), and also was detergent-soluble (Fig.  3g).	gene_phenotype
69051	5	333204	5	NULL	NULL	0	NULL	YPL176-GFP	GP	localization of	excluded from		mostly			shmoo tip	CellComponent				NULL		0	NULL	NULL	NULL	gw60_pnas_99_22_14183_s_101	12374868	A GFP fusion of yeast transferrin receptor-like YPL176c (YPL176-GFP) localized in a punctate pattern along the surface of the body of the cell, mostly excluded from the shmoo tip (Fig.  3 c), and also was detergent-soluble (Fig.  3g).	gene_phenotype
69052	1	333207	5	NULL	NULL	0	NULL	Ydr527wp protein	GP	Saccharomyces cerevisiae	is required for					cell viability	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_16_7043_s_151	15282305	In addition, these proteins show significant similarities to the  Saccharomyces cerevisiae Ydr527wp protein (accession no.  NP 010816), which is required for cell viability and was shown to bind the Rpb10 subunit of RNAPII in a two-hybrid screen ( ,  ).	gene_phenotype
69053	2	333207	5	NULL	NULL	0	NULL	Ydr527wp protein	GP	Saccharomyces cerevisiae	bind					RNAPII	GP		Rpb10 subunit		NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_16_7043_s_151	15282305	In addition, these proteins show significant similarities to the  Saccharomyces cerevisiae Ydr527wp protein (accession no.  NP 010816), which is required for cell viability and was shown to bind the Rpb10 subunit of RNAPII in a two-hybrid screen ( ,  ).	gene_phenotype
69054	1	333208	5	NULL	NULL	0	NULL	YGR156w	NucleicAcid		is the locus name of					PTI1	GP				NULL		0	NULL	NULL	NULL	gw60_molcell_10_6_1429_s_32	12504017	PTI1 (YGR156w) Is a Suppressor of  ctk1  Cold Sensitivity	gene_phenotype
69055	2	333208	5	NULL	NULL	0	NULL	ctk1	GP		is sensitive to					cold	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	gw60_molcell_10_6_1429_s_32	12504017	PTI1 (YGR156w) Is a Suppressor of  ctk1  Cold Sensitivity	gene_phenotype
69056	3	333208	5	NULL	NULL	0	NULL	PTI1	GP		is a suppressor of					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_10_6_1429_s_32	12504017	PTI1 (YGR156w) Is a Suppressor of  ctk1  Cold Sensitivity	gene_phenotype
69057	1	333210	5	NULL	NULL	0	NULL	yhl021c	NucleicAcid	mutant	does not show										NULL		0	NULL	NULL	NULL	gw60_genetics_155_4_1607_s_91	10924460	yhl021c mutants have no detectable phenotype in mitosis or meiosis.	gene_phenotype
69058	1	333211	5	NULL	NULL	NULL	NULL	haploid cells	Cell		contains					Ykl082c-YFP	GP	genomic			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_3_549_s_156	11489916	We found that haploid cells containing the genomic Ykl082c-YFP fusion were slow growing and temperature sensitive.	gene_phenotype
69059	2	333211	5	NULL	NULL	0	NULL	Ykl082c-YFP	GP		is a type of					fusion protein	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_154_3_549_s_156	11489916	We found that haploid cells containing the genomic Ykl082c-YFP fusion were slow growing and temperature sensitive.	gene_phenotype
69060	3	333211	5	NULL	NULL	0	NULL	statement 1	Process		shows					growth	Process	slow			NULL		0	NULL	NULL	NULL	gw60_cellbiol_154_3_549_s_156	11489916	We found that haploid cells containing the genomic Ykl082c-YFP fusion were slow growing and temperature sensitive.	gene_phenotype
69061	4	333211	5	NULL	NULL	0	NULL	statement 1	Process		is sensitive to					temperature	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	gw60_cellbiol_154_3_549_s_156	11489916	We found that haploid cells containing the genomic Ykl082c-YFP fusion were slow growing and temperature sensitive.	gene_phenotype
69062	1	333217	5	NULL	NULL	0	NULL	YNR039c	NucleicAcid		encodes					zinc transporter proteins	GP	potential			NULL		0	NULL	NULL	NULL	gw60_pnas_97_14_7957_s_202	10884426	Several other genes in our list of Zap1p targets also encode potential zinc transporter proteins including YNR039c and YOL002c.	gene_phenotype
69063	2	333217	5	NULL	NULL	0	NULL	YOL002c	NucleicAcid		encodes					zinc transporter proteins	GP	potential			NULL		0	NULL	NULL	NULL	gw60_pnas_97_14_7957_s_202	10884426	Several other genes in our list of Zap1p targets also encode potential zinc transporter proteins including YNR039c and YOL002c.	gene_phenotype
69064	1	333219	5	NULL	NULL	0	NULL	Ypl244c protein	GP		is similar to		most			UDP-Gal transporter	GP	S. pombe			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4424_s_272	11067855	The function of Ypl244c is unknown, although this protein is most similar to the  S. pombe UDP-Gal transporter and appears to be localized in the Golgi ( 16).	gene_phenotype
69065	2	333219	5	NULL	NULL	0	NULL	Ypl244c protein	GP		is localized in		appears to be			Golgi	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4424_s_272	11067855	The function of Ypl244c is unknown, although this protein is most similar to the  S. pombe UDP-Gal transporter and appears to be localized in the Golgi ( 16).	gene_phenotype
69066	1	333220	5	NULL	NULL	0	NULL	UDP-sugar transporter family	GP		does not contain							conserved	GALNK motif		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4424_s_270	11067855	Two  S. cerevisiae proteins, Yel004p and Ypl244c, were identified as members of the UDP-sugar transporter family that do not contain the conserved GALNK motif.	gene_phenotype
69067	2	333220	5	NULL	NULL	0	NULL	Yel004p protein	GP		is a member of					statement 1	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4424_s_270	11067855	Two  S. cerevisiae proteins, Yel004p and Ypl244c, were identified as members of the UDP-sugar transporter family that do not contain the conserved GALNK motif.	gene_phenotype
69068	3	333220	5	NULL	NULL	0	NULL	Ypl244c protein	GP		is a member of					statement 1	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4424_s_270	11067855	Two  S. cerevisiae proteins, Yel004p and Ypl244c, were identified as members of the UDP-sugar transporter family that do not contain the conserved GALNK motif.	gene_phenotype
69069	1	333222	5	NULL	NULL	0	NULL	Ybr001c	NucleicAcid		encodes for					Nth2	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_132	16498703	Ybr001c  Nth2  2 Putative neutral trehalase, required for thermotolerance and may mediate resistance  to other cellular stresses  LIP  [ 16]	gene_phenotype
69070	1	333222	5	NULL	NULL	0	NULL	Ybr001c	NucleicAcid		encodes for					Nth2	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_132	16498703	Ybr001c  Nth2  2 Putative neutral trehalase, required for thermotolerance and may mediate resistance  to other cellular stresses  LIP  [ 16]	gene_phenotype
69071	1	333222	5	NULL	NULL	0	NULL	Ybr001c	NucleicAcid		encodes for					Nth2	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_132	16498703	Ybr001c  Nth2  2 Putative neutral trehalase, required for thermotolerance and may mediate resistance  to other cellular stresses  LIP  [ 16]	gene_phenotype
69072	2	333222	5	NULL	NULL	0	NULL	Nth2	GP		is a synonym of					Putative neutral trehalase	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_132	16498703	Ybr001c  Nth2  2 Putative neutral trehalase, required for thermotolerance and may mediate resistance  to other cellular stresses  LIP  [ 16]	gene_phenotype
69073	3	333222	5	NULL	NULL	0	NULL	Nth2	GP		is required for					thermotolerance	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_132	16498703	Ybr001c  Nth2  2 Putative neutral trehalase, required for thermotolerance and may mediate resistance  to other cellular stresses  LIP  [ 16]	gene_phenotype
69074	4	333222	5	NULL	NULL	0	NULL	Nth2	GP		mediates		may			cellular stresses	Process	resistance to			NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_132	16498703	Ybr001c  Nth2  2 Putative neutral trehalase, required for thermotolerance and may mediate resistance  to other cellular stresses  LIP  [ 16]	gene_phenotype
69076	1	333223	5	NULL	NULL	0	NULL	YBR201W	NucleicAcid		encodes for					DER1	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_363	15334557	DER1   YBR201W Endoplasmic reticulum membrane protein, required for the protein degradation process  associated with the ER, involved in the retrograde transport of misfolded or unassembled  proteins	gene_phenotype
69077	2	333223	5	NULL	NULL	0	NULL	DER1	GP		is a type of					Endoplasmic reticulum membrane protein	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_363	15334557	DER1   YBR201W Endoplasmic reticulum membrane protein, required for the protein degradation process  associated with the ER, involved in the retrograde transport of misfolded or unassembled  proteins	gene_phenotype
69078	3	333223	5	NULL	NULL	0	NULL	protein degradation	Process		is associated with					ER	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_363	15334557	DER1   YBR201W Endoplasmic reticulum membrane protein, required for the protein degradation process  associated with the ER, involved in the retrograde transport of misfolded or unassembled  proteins	gene_phenotype
69079	4	333223	5	NULL	NULL	0	NULL	DER1	GP		is required for					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_363	15334557	DER1   YBR201W Endoplasmic reticulum membrane protein, required for the protein degradation process  associated with the ER, involved in the retrograde transport of misfolded or unassembled  proteins	gene_phenotype
69080	5	333223	5	NULL	NULL	0	NULL	proteins	GP	misfolded	undergoes					transport	Process	retrograde			NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_363	15334557	DER1   YBR201W Endoplasmic reticulum membrane protein, required for the protein degradation process  associated with the ER, involved in the retrograde transport of misfolded or unassembled  proteins	gene_phenotype
69081	6	333223	5	NULL	NULL	0	NULL	DER1	GP		is involved in					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_363	15334557	DER1   YBR201W Endoplasmic reticulum membrane protein, required for the protein degradation process  associated with the ER, involved in the retrograde transport of misfolded or unassembled  proteins	gene_phenotype
69082	7	333223	5	NULL	NULL	0	NULL	proteins	GP	unassembled	undergoes					transport	Process	retrograde			NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_363	15334557	DER1   YBR201W Endoplasmic reticulum membrane protein, required for the protein degradation process  associated with the ER, involved in the retrograde transport of misfolded or unassembled  proteins	gene_phenotype
69083	8	333223	5	NULL	NULL	0	NULL	DER1	GP		is involved in					statement 7	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_363	15334557	DER1   YBR201W Endoplasmic reticulum membrane protein, required for the protein degradation process  associated with the ER, involved in the retrograde transport of misfolded or unassembled  proteins	gene_phenotype
69084	9	333223	5	NULL	NULL	0	NULL	statement 5	Process		is an alternative to					statement 7	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_363	15334557	DER1   YBR201W Endoplasmic reticulum membrane protein, required for the protein degradation process  associated with the ER, involved in the retrograde transport of misfolded or unassembled  proteins	gene_phenotype
69085	1	333224	5	NULL	NULL	0	NULL	yhr101c	NucleicAcid		is the locus name of					big1	GP				NULL		0	NULL	NULL	NULL	gw60_science_285_5429_901_s_72	10436161	For example, the previously-constructed  yhr101c ( big1) and  ybr196c ( pgi1) null mutants show glucose sensitivity, and the  ybr256c ( rib5) deletion mutant requires a riboflavin supplement for viability ( 24).	gene_phenotype
69086	2	333224	5	NULL	NULL	0	NULL	ybr196c	NucleicAcid		is the locus name of					pgi1	GP				NULL		0	NULL	NULL	NULL	gw60_science_285_5429_901_s_72	10436161	For example, the previously-constructed  yhr101c ( big1) and  ybr196c ( pgi1) null mutants show glucose sensitivity, and the  ybr256c ( rib5) deletion mutant requires a riboflavin supplement for viability ( 24).	gene_phenotype
69087	3	333224	5	NULL	NULL	0	NULL	ybr256c	NucleicAcid		is the locus name of					rib5	GP				NULL		0	NULL	NULL	NULL	gw60_science_285_5429_901_s_72	10436161	For example, the previously-constructed  yhr101c ( big1) and  ybr196c ( pgi1) null mutants show glucose sensitivity, and the  ybr256c ( rib5) deletion mutant requires a riboflavin supplement for viability ( 24).	gene_phenotype
69088	4	333224	5	NULL	NULL	0	NULL	yhr101c	NucleicAcid	null mutant	is sensitive to					glucose	Chemical				NULL		0	NULL	NULL	NULL	gw60_science_285_5429_901_s_72	10436161	For example, the previously-constructed  yhr101c ( big1) and  ybr196c ( pgi1) null mutants show glucose sensitivity, and the  ybr256c ( rib5) deletion mutant requires a riboflavin supplement for viability ( 24).	gene_phenotype
69089	5	333224	5	NULL	NULL	0	NULL	ybr196c	NucleicAcid	null mutant	is sensitive to					glucose	Chemical				NULL		0	NULL	NULL	NULL	gw60_science_285_5429_901_s_72	10436161	For example, the previously-constructed  yhr101c ( big1) and  ybr196c ( pgi1) null mutants show glucose sensitivity, and the  ybr256c ( rib5) deletion mutant requires a riboflavin supplement for viability ( 24).	gene_phenotype
69090	6	333224	5	NULL	NULL	0	NULL	riboflavin supplement	Chemical		is required for					viability	Process				NULL		0	NULL	NULL	NULL	gw60_science_285_5429_901_s_72	10436161	For example, the previously-constructed  yhr101c ( big1) and  ybr196c ( pgi1) null mutants show glucose sensitivity, and the  ybr256c ( rib5) deletion mutant requires a riboflavin supplement for viability ( 24).	gene_phenotype
69091	7	333224	5	NULL	NULL	0	NULL	ybr256c	NucleicAcid	deletion mutant	requires					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_science_285_5429_901_s_72	10436161	For example, the previously-constructed  yhr101c ( big1) and  ybr196c ( pgi1) null mutants show glucose sensitivity, and the  ybr256c ( rib5) deletion mutant requires a riboflavin supplement for viability ( 24).	gene_phenotype
69092	1	333225	5	NULL	NULL	0	NULL	YCR002c	NucleicAcid		is the locus name of					CDC10	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_285	15334557	CDC10   YCR002c Component of septin ring of the mother-bud neck; required for cytokinesis	gene_phenotype
69093	2	333225	5	NULL	NULL	0	NULL	CDC10	GP		is a component of					mother-bud neck	CellComponent	septin ring of			NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_285	15334557	CDC10   YCR002c Component of septin ring of the mother-bud neck; required for cytokinesis	gene_phenotype
69094	3	333225	5	NULL	NULL	0	NULL	CDC10	GP		is required for					cytokinesis	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_285	15334557	CDC10   YCR002c Component of septin ring of the mother-bud neck; required for cytokinesis	gene_phenotype
67978	1	333228	7	NULL	NULL	0	NULL	Ycr072c	GP		is required for					cell	Cell	viability of			NULL		0	NULL	NULL	NULL	gw70_nature_435_7043_814_s_82	15944704	For the protein Ycr072c, which is required for the viability of the cell and appears  in the dark green community on the right, SGD provides no biological process (function).	gene_phenotype
68041	1	333231	7	NULL	NULL	NULL	NULL	Ydr001c Nth1 1, 2 Neutral trehalase	GP		degrades					trehalose	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_yeast_23_3_159_s_131	16498703	Ydr001c  Nth1 1, 2 Neutral trehalase, degrades trehalose; required for thermotolerance and may mediate  resistance to other cellular stresses; may be phosphorylated by Cdc28p  LIP  [ 16],[ 20]	gene_phenotype
68042	2	333231	7	NULL	NULL	0	NULL	trehalose	Chemical		required for					thermotolerance	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_131	16498703	Ydr001c  Nth1 1, 2 Neutral trehalase, degrades trehalose; required for thermotolerance and may mediate  resistance to other cellular stresses; may be phosphorylated by Cdc28p  LIP  [ 16],[ 20]	gene_phenotype
68043	3	333231	7	NULL	NULL	NULL	NULL	Ydr001c Nth1 1, 2 Neutral trehalase	GP		mediate		may			cellular stress	Process	resistance to			NULL		NULL	NULL	NULL	NULL	gw70_yeast_23_3_159_s_131	16498703	Ydr001c  Nth1 1, 2 Neutral trehalase, degrades trehalose; required for thermotolerance and may mediate  resistance to other cellular stresses; may be phosphorylated by Cdc28p  LIP  [ 16],[ 20]	gene_phenotype
68044	4	333231	7	NULL	NULL	NULL	NULL	Cdc28p LIP	GP		phosphorylate					Ydr001c Nth1 1, 2 Neutral trehalase	GP				NULL		NULL	NULL	NULL	NULL	gw70_yeast_23_3_159_s_131	16498703	Ydr001c  Nth1 1, 2 Neutral trehalase, degrades trehalose; required for thermotolerance and may mediate  resistance to other cellular stresses; may be phosphorylated by Cdc28p  LIP  [ 16],[ 20]	gene_phenotype
68045	1	333232	7	NULL	NULL	NULL	NULL	Ydr006c Sok1 1 Protein	GP	overexpression of	suppresses					growth defect	Process				NULL	mutants lacking protein kinase A activity	NULL	NULL	NULL	NULL	gw70_yeast_23_3_159_s_136	16498703	Ydr006c  Sok1  1 Protein whose overexpression suppresses the growth defect of mutants lacking protein  kinase A activity; involved in cAMP-mediated signalling; localized to the nucleus;  similar to the mouse testis-specific protein PBS13  LIP  [ 20]	gene_phenotype
68046	2	333232	7	NULL	NULL	0	NULL	cAMP	Chemical		mediates					signal	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_136	16498703	Ydr006c  Sok1  1 Protein whose overexpression suppresses the growth defect of mutants lacking protein  kinase A activity; involved in cAMP-mediated signalling; localized to the nucleus;  similar to the mouse testis-specific protein PBS13  LIP  [ 20]	gene_phenotype
68047	4	333232	7	NULL	NULL	NULL	NULL	Ydr006c Sok1 1 Protein	GP		localized to					nucleus	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_yeast_23_3_159_s_136	16498703	Ydr006c  Sok1  1 Protein whose overexpression suppresses the growth defect of mutants lacking protein  kinase A activity; involved in cAMP-mediated signalling; localized to the nucleus;  similar to the mouse testis-specific protein PBS13  LIP  [ 20]	gene_phenotype
68048	3	333232	7	NULL	NULL	0	NULL	Ydr006c Sok1 1 Protein	GP		involved in					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_136	16498703	Ydr006c  Sok1  1 Protein whose overexpression suppresses the growth defect of mutants lacking protein  kinase A activity; involved in cAMP-mediated signalling; localized to the nucleus;  similar to the mouse testis-specific protein PBS13  LIP  [ 20]	gene_phenotype
68049	5	333232	7	NULL	NULL	0	NULL	testis-specific protein PBS13 LIP	GP	mouse;;overexpression of	suppresses					growth defect	Process				NULL	mutants lacking protein kinase A activity	0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_136	16498703	Ydr006c  Sok1  1 Protein whose overexpression suppresses the growth defect of mutants lacking protein  kinase A activity; involved in cAMP-mediated signalling; localized to the nucleus;  similar to the mouse testis-specific protein PBS13  LIP  [ 20]	gene_phenotype
68050	6	333232	7	NULL	NULL	0	NULL	testis-specific protein PBS13 LIP	GP	mouse	involved in					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_136	16498703	Ydr006c  Sok1  1 Protein whose overexpression suppresses the growth defect of mutants lacking protein  kinase A activity; involved in cAMP-mediated signalling; localized to the nucleus;  similar to the mouse testis-specific protein PBS13  LIP  [ 20]	gene_phenotype
68051	7	333232	7	NULL	NULL	0	NULL	testis-specific protein PBS13 LIP	GP	mouse	localized to					nucleus	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_136	16498703	Ydr006c  Sok1  1 Protein whose overexpression suppresses the growth defect of mutants lacking protein  kinase A activity; involved in cAMP-mediated signalling; localized to the nucleus;  similar to the mouse testis-specific protein PBS13  LIP  [ 20]	gene_phenotype
68052	8	333232	7	NULL	NULL	0	NULL	statement 1	Process		is similar to					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_136	16498703	Ydr006c  Sok1  1 Protein whose overexpression suppresses the growth defect of mutants lacking protein  kinase A activity; involved in cAMP-mediated signalling; localized to the nucleus;  similar to the mouse testis-specific protein PBS13  LIP  [ 20]	gene_phenotype
68053	9	333232	7	NULL	NULL	0	NULL	statement 3	Process		is similar to					statement 6	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_136	16498703	Ydr006c  Sok1  1 Protein whose overexpression suppresses the growth defect of mutants lacking protein  kinase A activity; involved in cAMP-mediated signalling; localized to the nucleus;  similar to the mouse testis-specific protein PBS13  LIP  [ 20]	gene_phenotype
68054	10	333232	7	NULL	NULL	0	NULL	statement 4	Process		is similar to					statement 7	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_136	16498703	Ydr006c  Sok1  1 Protein whose overexpression suppresses the growth defect of mutants lacking protein  kinase A activity; involved in cAMP-mediated signalling; localized to the nucleus;  similar to the mouse testis-specific protein PBS13  LIP  [ 20]	gene_phenotype
68055	1	333233	7	NULL	NULL	0	NULL	Cdc7p-Dbf4p kinase complex	GP		required for			YDR052c DBF4 Regulatory subunit		Cdc7p kinase	GP	 activity of			NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_83	16498703	YDR052c   DBF4 Regulatory subunit of Cdc7p-Dbf4p kinase complex, required for Cdc7p kinase activity  and initiation of DNA replication; phosphorylates the Mcm2-7 family of proteins;  cell cycle-regulated  [ 49]	gene_phenotype
68056	2	333233	7	NULL	NULL	0	NULL	Cdc7p-Dbf4p kinase complex	GP		initiates			YDR052c DBF4 Regulatory subunit		DNA replication	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_83	16498703	YDR052c   DBF4 Regulatory subunit of Cdc7p-Dbf4p kinase complex, required for Cdc7p kinase activity  and initiation of DNA replication; phosphorylates the Mcm2-7 family of proteins;  cell cycle-regulated  [ 49]	gene_phenotype
68057	3	333233	7	NULL	NULL	0	NULL	Cdc7p-Dbf4p kinase complex	GP		phosphorylates			YDR052c DBF4 Regulatory subunit		Mcm2-7 family	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_83	16498703	YDR052c   DBF4 Regulatory subunit of Cdc7p-Dbf4p kinase complex, required for Cdc7p kinase activity  and initiation of DNA replication; phosphorylates the Mcm2-7 family of proteins;  cell cycle-regulated  [ 49]	gene_phenotype
68058	1	333234	7	NULL	NULL	0	NULL	NUM1 YDR150w Tubulin	GP		function		may			nuclear migration	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_218	15334557	NUM1   YDR150w Tubulin binding; may function in nuclear migration during mitosis and meiosis by affecting  astral microtubule functions, perhaps by being involved in polymerization and stabilization  of microtubules	gene_phenotype
68059	2	333234	7	NULL	NULL	0	NULL	statement 1	Process		occur during					mitosis	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_218	15334557	NUM1   YDR150w Tubulin binding; may function in nuclear migration during mitosis and meiosis by affecting  astral microtubule functions, perhaps by being involved in polymerization and stabilization  of microtubules	gene_phenotype
68060	3	333234	7	NULL	NULL	0	NULL	statement 1	Process		occur during					meiosis	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_218	15334557	NUM1   YDR150w Tubulin binding; may function in nuclear migration during mitosis and meiosis by affecting  astral microtubule functions, perhaps by being involved in polymerization and stabilization  of microtubules	gene_phenotype
68061	4	333234	7	NULL	NULL	NULL	NULL	statement 1	Process		occur by					astral microtubule functions	Process	affecting			NULL		NULL	NULL	NULL	NULL	gw70_yeast_21_11_927_s_218	15334557	NUM1   YDR150w Tubulin binding; may function in nuclear migration during mitosis and meiosis by affecting  astral microtubule functions, perhaps by being involved in polymerization and stabilization  of microtubules	gene_phenotype
68062	6	333234	7	NULL	NULL	NULL	NULL	statement 1	Process		affect					 microtubules	Chromosome	stabilization of			NULL		NULL	NULL	NULL	NULL	gw70_yeast_21_11_927_s_218	15334557	NUM1   YDR150w Tubulin binding; may function in nuclear migration during mitosis and meiosis by affecting  astral microtubule functions, perhaps by being involved in polymerization and stabilization  of microtubules	gene_phenotype
68063	5	333234	7	NULL	NULL	NULL	NULL	statement 1	Process		affect					microtubules	Chromosome	polymerization of			NULL		NULL	NULL	NULL	NULL	gw70_yeast_21_11_927_s_218	15334557	NUM1   YDR150w Tubulin binding; may function in nuclear migration during mitosis and meiosis by affecting  astral microtubule functions, perhaps by being involved in polymerization and stabilization  of microtubules	gene_phenotype
68064	7	333234	7	NULL	NULL	0	NULL	statement 4	Process		involves					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_218	15334557	NUM1   YDR150w Tubulin binding; may function in nuclear migration during mitosis and meiosis by affecting  astral microtubule functions, perhaps by being involved in polymerization and stabilization  of microtubules	gene_phenotype
68065	8	333234	7	NULL	NULL	0	NULL	statement 5	Process		involves					statement 6	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_218	15334557	NUM1   YDR150w Tubulin binding; may function in nuclear migration during mitosis and meiosis by affecting  astral microtubule functions, perhaps by being involved in polymerization and stabilization  of microtubules	gene_phenotype
68066	1	333235	7	NULL	NULL	0	NULL	SAC3 YDR159w Nuclear pore 	CellComponent	component of	involved in					mRNA	NucleicAcid	nuclear export of			NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_203	15334557	SAC3   YDR159w Nuclear pore component; involved in nuclear export of both mRNA and protein	gene_phenotype
68067	2	333235	7	NULL	NULL	NULL	NULL	SAC3 YDR159w Nuclear pore 	CellComponent	component of	involved in					protein	GP	nuclear export of			NULL		NULL	NULL	NULL	NULL	gw70_yeast_21_11_927_s_203	15334557	SAC3   YDR159w Nuclear pore component; involved in nuclear export of both mRNA and protein	gene_phenotype
68068	1	333236	7	NULL	NULL	0	NULL	YDR227W SIR4	GP		is a type of					silencing regulator	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_20_9_827_s_119	12845608	YDR227W   SIR4 Silencing regulator  2.0	gene_phenotype
68069	1	333239	7	NULL	NULL	0	NULL	YEL061c CIN8 Kinesin motor protein	GP		involved in					mitotic spindle assembly	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_84	16498703	YEL061c   CIN8 Kinesin motor protein involved in mitotic spindle assembly and chromosome segregation  [ 49]	gene_phenotype
68070	2	333239	7	NULL	NULL	0	NULL	YEL061c CIN8 Kinesin motor protein	GP		involved in					chromosome segregation	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_84	16498703	YEL061c   CIN8 Kinesin motor protein involved in mitotic spindle assembly and chromosome segregation  [ 49]	gene_phenotype
68071	1	333240	7	NULL	NULL	0	NULL	YER075c PTP3	GP		downregulate					Hog1p	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_19_7_587_s_67	11967829	YER075c   PTP3 Downregulate Hog1p and Fus3p MAPK, sporulation (Maeda  et al., [ 1994]; Wurgler-Murphy  et al., [ 1997]; Zhan  et al., [ 2000])	gene_phenotype
68072	2	333240	7	NULL	NULL	0	NULL	YER075c PTP3	GP		downregulates					Fus3p MAPK	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_19_7_587_s_67	11967829	YER075c   PTP3 Downregulate Hog1p and Fus3p MAPK, sporulation (Maeda  et al., [ 1994]; Wurgler-Murphy  et al., [ 1997]; Zhan  et al., [ 2000])	gene_phenotype
68073	1	333242	7	NULL	NULL	0	NULL	YGL001c 	GP	disruption of	viable in					hem 1delta strain	Organism				NULL		0	NULL	NULL	NULL	gw60_pnas_95_23_13794_s_8	9811880	The YGL001c (  ERG26) disruption also was viable in a   hem 1delta strain grown in the presence of ergosterol.	gene_phenotype
68074	2	333242	7	NULL	NULL	0	NULL	hem 1delta strain	Organism		grown					ergosterol	Chemical	in the presence of			NULL		0	NULL	NULL	NULL	gw60_pnas_95_23_13794_s_8	9811880	The YGL001c (  ERG26) disruption also was viable in a   hem 1delta strain grown in the presence of ergosterol.	gene_phenotype
68075	3	333242	7	NULL	NULL	0	NULL	YGL001c 	GP		is					ERG26	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_95_23_13794_s_8	9811880	The YGL001c (  ERG26) disruption also was viable in a   hem 1delta strain grown in the presence of ergosterol.	gene_phenotype
68076	1	333244	7	NULL	NULL	0	NULL	one segregant	Organism		derived from					SDG274	Organism				NULL		0	NULL	NULL	NULL	gw60_pnas_95_23_13794_s_104	9811880	However, one segregant derived from SDG274, SDG 274-6, was able to grow both aerobically and anaerobically on ergosterol media, suggesting that disruption of YGL001c gives rise to sterol auxotrophy and that a second mutation may have arisen in this strain.	gene_phenotype
68077	2	333244	7	NULL	NULL	0	NULL	one segregant	Organism		derived from					SDG 274-6	Organism				NULL		0	NULL	NULL	NULL	gw60_pnas_95_23_13794_s_104	9811880	However, one segregant derived from SDG274, SDG 274-6, was able to grow both aerobically and anaerobically on ergosterol media, suggesting that disruption of YGL001c gives rise to sterol auxotrophy and that a second mutation may have arisen in this strain.	gene_phenotype
68078	3	333244	7	NULL	NULL	NULL	NULL	statement 1	Organism		grow					aerobically	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_23_13794_s_104	9811880	However, one segregant derived from SDG274, SDG 274-6, was able to grow both aerobically and anaerobically on ergosterol media, suggesting that disruption of YGL001c gives rise to sterol auxotrophy and that a second mutation may have arisen in this strain.	gene_phenotype
68079	4	333244	7	NULL	NULL	NULL	NULL	statement 1	Organism		grow					anaerobically	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_23_13794_s_104	9811880	However, one segregant derived from SDG274, SDG 274-6, was able to grow both aerobically and anaerobically on ergosterol media, suggesting that disruption of YGL001c gives rise to sterol auxotrophy and that a second mutation may have arisen in this strain.	gene_phenotype
68080	5	333244	7	NULL	NULL	0	NULL	statement 2	Organism		grow					aerobically	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_95_23_13794_s_104	9811880	However, one segregant derived from SDG274, SDG 274-6, was able to grow both aerobically and anaerobically on ergosterol media, suggesting that disruption of YGL001c gives rise to sterol auxotrophy and that a second mutation may have arisen in this strain.	gene_phenotype
68081	6	333244	7	NULL	NULL	0	NULL	statement 2	Organism		grow					anaerobically	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_95_23_13794_s_104	9811880	However, one segregant derived from SDG274, SDG 274-6, was able to grow both aerobically and anaerobically on ergosterol media, suggesting that disruption of YGL001c gives rise to sterol auxotrophy and that a second mutation may have arisen in this strain.	gene_phenotype
68082	7	333244	7	NULL	NULL	NULL	NULL	statement 3	Process		grown on					ergosterol media	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_23_13794_s_104	9811880	However, one segregant derived from SDG274, SDG 274-6, was able to grow both aerobically and anaerobically on ergosterol media, suggesting that disruption of YGL001c gives rise to sterol auxotrophy and that a second mutation may have arisen in this strain.	gene_phenotype
68083	8	333244	7	NULL	NULL	0	NULL	statement 4	Process		grown on					ergosterol media	Chemical				NULL		0	NULL	NULL	NULL	gw60_pnas_95_23_13794_s_104	9811880	However, one segregant derived from SDG274, SDG 274-6, was able to grow both aerobically and anaerobically on ergosterol media, suggesting that disruption of YGL001c gives rise to sterol auxotrophy and that a second mutation may have arisen in this strain.	gene_phenotype
68084	9	333244	7	NULL	NULL	0	NULL	statement 5	Process		grown on					ergosterol media	Chemical				NULL		0	NULL	NULL	NULL	gw60_pnas_95_23_13794_s_104	9811880	However, one segregant derived from SDG274, SDG 274-6, was able to grow both aerobically and anaerobically on ergosterol media, suggesting that disruption of YGL001c gives rise to sterol auxotrophy and that a second mutation may have arisen in this strain.	gene_phenotype
68085	10	333244	7	NULL	NULL	0	NULL	statement 6	Process		grown on					ergosterol media	Chemical				NULL		0	NULL	NULL	NULL	gw60_pnas_95_23_13794_s_104	9811880	However, one segregant derived from SDG274, SDG 274-6, was able to grow both aerobically and anaerobically on ergosterol media, suggesting that disruption of YGL001c gives rise to sterol auxotrophy and that a second mutation may have arisen in this strain.	gene_phenotype
68086	11	333244	7	NULL	NULL	0	NULL	YGL001c	GP	disruption of	gives rise to					sterol auxotrophy	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_95_23_13794_s_104	9811880	However, one segregant derived from SDG274, SDG 274-6, was able to grow both aerobically and anaerobically on ergosterol media, suggesting that disruption of YGL001c gives rise to sterol auxotrophy and that a second mutation may have arisen in this strain.	gene_phenotype
68087	12	333244	7	NULL	NULL	0	NULL	statement 3	Process		suggests					statement 11	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_95_23_13794_s_104	9811880	However, one segregant derived from SDG274, SDG 274-6, was able to grow both aerobically and anaerobically on ergosterol media, suggesting that disruption of YGL001c gives rise to sterol auxotrophy and that a second mutation may have arisen in this strain.	gene_phenotype
68088	13	333244	7	NULL	NULL	0	NULL	statement 4	Process		suggests					statement 11	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_95_23_13794_s_104	9811880	However, one segregant derived from SDG274, SDG 274-6, was able to grow both aerobically and anaerobically on ergosterol media, suggesting that disruption of YGL001c gives rise to sterol auxotrophy and that a second mutation may have arisen in this strain.	gene_phenotype
68089	14	333244	7	NULL	NULL	0	NULL	statement 5	Process		suggests					statement 11	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_95_23_13794_s_104	9811880	However, one segregant derived from SDG274, SDG 274-6, was able to grow both aerobically and anaerobically on ergosterol media, suggesting that disruption of YGL001c gives rise to sterol auxotrophy and that a second mutation may have arisen in this strain.	gene_phenotype
68090	15	333244	7	NULL	NULL	0	NULL	statement 6	Process		suggests					statement 11	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_95_23_13794_s_104	9811880	However, one segregant derived from SDG274, SDG 274-6, was able to grow both aerobically and anaerobically on ergosterol media, suggesting that disruption of YGL001c gives rise to sterol auxotrophy and that a second mutation may have arisen in this strain.	gene_phenotype
68176	4	333245	7	NULL	NULL	NULL	NULL	Ygl115w Snf4 1 Protein kinase activator	GP		involved in					glucose-repressed genes	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_yeast_23_3_159_s_126	16498703	Ygl115w  Snf4  1 Protein kinase activator found in a complex containing Snf1p and members of the Sip1p/Sip2p/Gal83p  family; activates the Snf1p protein kinase; involved in expression of glucose-repressed  genes, sporulation and peroxisome biogenesis  LIP  [ 16]	gene_phenotype
68177	3	333245	7	NULL	NULL	NULL	NULL	Ygl115w Snf4 1 Protein kinase activator	GP		activates					Snf1p protein kinase	GP				NULL		NULL	NULL	NULL	NULL	gw70_yeast_23_3_159_s_126	16498703	Ygl115w  Snf4  1 Protein kinase activator found in a complex containing Snf1p and members of the Sip1p/Sip2p/Gal83p  family; activates the Snf1p protein kinase; involved in expression of glucose-repressed  genes, sporulation and peroxisome biogenesis  LIP  [ 16]	gene_phenotype
68178	5	333245	7	NULL	NULL	NULL	NULL	Ygl115w Snf4 1 Protein kinase activator	GP		involved in					sporulation	Process	expression of			NULL		NULL	NULL	NULL	NULL	gw70_yeast_23_3_159_s_126	16498703	Ygl115w  Snf4  1 Protein kinase activator found in a complex containing Snf1p and members of the Sip1p/Sip2p/Gal83p  family; activates the Snf1p protein kinase; involved in expression of glucose-repressed  genes, sporulation and peroxisome biogenesis  LIP  [ 16]	gene_phenotype
68179	6	333245	7	NULL	NULL	NULL	NULL	Ygl115w Snf4 1 Protein kinase activator	GP		involved in					peroxisome	CellComponent	expression of;;biogenesis of			NULL		NULL	NULL	NULL	NULL	gw70_yeast_23_3_159_s_126	16498703	Ygl115w  Snf4  1 Protein kinase activator found in a complex containing Snf1p and members of the Sip1p/Sip2p/Gal83p  family; activates the Snf1p protein kinase; involved in expression of glucose-repressed  genes, sporulation and peroxisome biogenesis  LIP  [ 16]	gene_phenotype
68181	1	333245	7	NULL	NULL	NULL	NULL	 Snf1p 	GP		in complex with					 Sip1p/Sip2p/Gal83p family	GP				NULL		NULL	NULL	NULL	NULL	gw70_yeast_23_3_159_s_126	16498703	Ygl115w  Snf4  1 Protein kinase activator found in a complex containing Snf1p and members of the Sip1p/Sip2p/Gal83p  family; activates the Snf1p protein kinase; involved in expression of glucose-repressed  genes, sporulation and peroxisome biogenesis  LIP  [ 16]	gene_phenotype
68182	2	333245	7	NULL	NULL	0	NULL	Ygl115w Snf4 1 Protein kinase activator	GP		found in					statement 1	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_126	16498703	Ygl115w  Snf4  1 Protein kinase activator found in a complex containing Snf1p and members of the Sip1p/Sip2p/Gal83p  family; activates the Snf1p protein kinase; involved in expression of glucose-repressed  genes, sporulation and peroxisome biogenesis  LIP  [ 16]	gene_phenotype
68183	1	333246	7	NULL	NULL	0	NULL	ymr308c ( PSE1)	GP		is a type of					haploid null mutant	GP				NULL		0	NULL	NULL	NULL	gw60_science_285_5429_901_s_73	10436161	In several cases, haploid null mutants were reported to have slow-growth phenotypes [ ymr308c ( PSE1),  yol022c,  ypl243c ( srp68),  ypl210c ( srp72), and  ydr353w ( trr1) ( 25)] or to be temperature sensitive [ ydr113c ( pds1) and  ygr216c ( gpi1) ( 26)].	gene_phenotype
68184	2	333246	7	NULL	NULL	0	NULL	yol022c	GP		is a type of					haploid null mutant	GP				NULL		0	NULL	NULL	NULL	gw60_science_285_5429_901_s_73	10436161	In several cases, haploid null mutants were reported to have slow-growth phenotypes [ ymr308c ( PSE1),  yol022c,  ypl243c ( srp68),  ypl210c ( srp72), and  ydr353w ( trr1) ( 25)] or to be temperature sensitive [ ydr113c ( pds1) and  ygr216c ( gpi1) ( 26)].	gene_phenotype
68185	3	333246	7	NULL	NULL	0	NULL	 ypl243c ( srp68)	GP		is a type of					haploid null mutant	GP				NULL		0	NULL	NULL	NULL	gw60_science_285_5429_901_s_73	10436161	In several cases, haploid null mutants were reported to have slow-growth phenotypes [ ymr308c ( PSE1),  yol022c,  ypl243c ( srp68),  ypl210c ( srp72), and  ydr353w ( trr1) ( 25)] or to be temperature sensitive [ ydr113c ( pds1) and  ygr216c ( gpi1) ( 26)].	gene_phenotype
68186	4	333246	7	NULL	NULL	0	NULL	ypl210c ( srp72)	GP		is a type of					haploid null mutant	GP				NULL		0	NULL	NULL	NULL	gw60_science_285_5429_901_s_73	10436161	In several cases, haploid null mutants were reported to have slow-growth phenotypes [ ymr308c ( PSE1),  yol022c,  ypl243c ( srp68),  ypl210c ( srp72), and  ydr353w ( trr1) ( 25)] or to be temperature sensitive [ ydr113c ( pds1) and  ygr216c ( gpi1) ( 26)].	gene_phenotype
68187	5	333246	7	NULL	NULL	0	NULL	ydr353w ( trr1)	GP		is a type of					haploid null mutant	GP				NULL		0	NULL	NULL	NULL	gw60_science_285_5429_901_s_73	10436161	In several cases, haploid null mutants were reported to have slow-growth phenotypes [ ymr308c ( PSE1),  yol022c,  ypl243c ( srp68),  ypl210c ( srp72), and  ydr353w ( trr1) ( 25)] or to be temperature sensitive [ ydr113c ( pds1) and  ygr216c ( gpi1) ( 26)].	gene_phenotype
68188	6	333246	7	NULL	NULL	0	NULL	statement 1	GP		possess					slow-growth phenotype	Process				NULL		0	NULL	NULL	NULL	gw60_science_285_5429_901_s_73	10436161	In several cases, haploid null mutants were reported to have slow-growth phenotypes [ ymr308c ( PSE1),  yol022c,  ypl243c ( srp68),  ypl210c ( srp72), and  ydr353w ( trr1) ( 25)] or to be temperature sensitive [ ydr113c ( pds1) and  ygr216c ( gpi1) ( 26)].	gene_phenotype
68189	7	333246	7	NULL	NULL	0	NULL	statement 2	GP		possess					slow-growth phenotype	Process				NULL		0	NULL	NULL	NULL	gw60_science_285_5429_901_s_73	10436161	In several cases, haploid null mutants were reported to have slow-growth phenotypes [ ymr308c ( PSE1),  yol022c,  ypl243c ( srp68),  ypl210c ( srp72), and  ydr353w ( trr1) ( 25)] or to be temperature sensitive [ ydr113c ( pds1) and  ygr216c ( gpi1) ( 26)].	gene_phenotype
68190	8	333246	7	NULL	NULL	0	NULL	statement 3	GP		possess					slow-growth phenotype	Process				NULL		0	NULL	NULL	NULL	gw60_science_285_5429_901_s_73	10436161	In several cases, haploid null mutants were reported to have slow-growth phenotypes [ ymr308c ( PSE1),  yol022c,  ypl243c ( srp68),  ypl210c ( srp72), and  ydr353w ( trr1) ( 25)] or to be temperature sensitive [ ydr113c ( pds1) and  ygr216c ( gpi1) ( 26)].	gene_phenotype
68191	9	333246	7	NULL	NULL	NULL	NULL	statement 4	GP		possess					slow-growth phenotype	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_285_5429_901_s_73	10436161	In several cases, haploid null mutants were reported to have slow-growth phenotypes [ ymr308c ( PSE1),  yol022c,  ypl243c ( srp68),  ypl210c ( srp72), and  ydr353w ( trr1) ( 25)] or to be temperature sensitive [ ydr113c ( pds1) and  ygr216c ( gpi1) ( 26)].	gene_phenotype
68192	10	333246	7	NULL	NULL	0	NULL	statement 5	GP		possess					slow-growth phenotype	Process				NULL		0	NULL	NULL	NULL	gw60_science_285_5429_901_s_73	10436161	In several cases, haploid null mutants were reported to have slow-growth phenotypes [ ymr308c ( PSE1),  yol022c,  ypl243c ( srp68),  ypl210c ( srp72), and  ydr353w ( trr1) ( 25)] or to be temperature sensitive [ ydr113c ( pds1) and  ygr216c ( gpi1) ( 26)].	gene_phenotype
68193	11	333246	7	NULL	NULL	0	NULL	ydr113c ( pds1)	GP		is a type of					haploid null mutant	GP				NULL		0	NULL	NULL	NULL	gw60_science_285_5429_901_s_73	10436161	In several cases, haploid null mutants were reported to have slow-growth phenotypes [ ymr308c ( PSE1),  yol022c,  ypl243c ( srp68),  ypl210c ( srp72), and  ydr353w ( trr1) ( 25)] or to be temperature sensitive [ ydr113c ( pds1) and  ygr216c ( gpi1) ( 26)].	gene_phenotype
68194	12	333246	7	NULL	NULL	0	NULL	 ygr216c ( gpi1)	GP		is a type of					haploid null mutant	GP				NULL		0	NULL	NULL	NULL	gw60_science_285_5429_901_s_73	10436161	In several cases, haploid null mutants were reported to have slow-growth phenotypes [ ymr308c ( PSE1),  yol022c,  ypl243c ( srp68),  ypl210c ( srp72), and  ydr353w ( trr1) ( 25)] or to be temperature sensitive [ ydr113c ( pds1) and  ygr216c ( gpi1) ( 26)].	gene_phenotype
68195	13	333246	7	NULL	NULL	0	NULL	statement 11	GP		is sensitive to					temperature	Process				NULL		0	NULL	NULL	NULL	gw60_science_285_5429_901_s_73	10436161	In several cases, haploid null mutants were reported to have slow-growth phenotypes [ ymr308c ( PSE1),  yol022c,  ypl243c ( srp68),  ypl210c ( srp72), and  ydr353w ( trr1) ( 25)] or to be temperature sensitive [ ydr113c ( pds1) and  ygr216c ( gpi1) ( 26)].	gene_phenotype
68196	14	333246	7	NULL	NULL	0	NULL	statement 12	GP		is sensitive to					temperature	Process				NULL		0	NULL	NULL	NULL	gw60_science_285_5429_901_s_73	10436161	In several cases, haploid null mutants were reported to have slow-growth phenotypes [ ymr308c ( PSE1),  yol022c,  ypl243c ( srp68),  ypl210c ( srp72), and  ydr353w ( trr1) ( 25)] or to be temperature sensitive [ ydr113c ( pds1) and  ygr216c ( gpi1) ( 26)].	gene_phenotype
68197	1	333247	7	NULL	NULL	NULL	NULL	ORF YHR105w 	GP	cells deleted for	shows					morphology		no defects in			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_140_3_577_s_150	9456318	A  null mutant of this gene was constructed, but cells deleted  for ORF YHR105w showed no defects in morphology,  vacuolar protein sorting, or Golgi membrane protein retention (data not shown).	gene_phenotype
68198	2	333247	7	NULL	NULL	NULL	NULL	ORF YHR105w 	GP	cells deleted for	shows					vacuolar protein	GP	no defects in sorting of			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_140_3_577_s_150	9456318	A  null mutant of this gene was constructed, but cells deleted  for ORF YHR105w showed no defects in morphology,  vacuolar protein sorting, or Golgi membrane protein retention (data not shown).	gene_phenotype
68199	3	333247	7	NULL	NULL	NULL	NULL	ORF YHR105w 	GP	cells deleted for	shows					 Golgi membrane protein 	GP	no defects in retention of			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_140_3_577_s_150	9456318	A  null mutant of this gene was constructed, but cells deleted  for ORF YHR105w showed no defects in morphology,  vacuolar protein sorting, or Golgi membrane protein retention (data not shown).	gene_phenotype
68200	1	333248	7	NULL	NULL	0	NULL	YHR171w	GP		is identified as					APG7	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_10_5_1353_s_228	10233149	YHR171w has recently been characterized and identified as  APG7, a gene required for nitrogen-starvation-induced autophagy in  S. cerevisiae (Tanida,  et al., 1999  ), as well as  CVT2, a gene necessary for constitutive delivery of pro-API from the cytosol to the vacuole by autophagy in  S. cerevisiae (Kim,  et al., 1999  ).	gene_phenotype
68201	2	333248	7	NULL	NULL	0	NULL	nitrogen-starvation	Process		induce					autophagy	Process				NULL	S. cerevisiae	0	NULL	NULL	NULL	gw60_molbiolcell_10_5_1353_s_228	10233149	YHR171w has recently been characterized and identified as  APG7, a gene required for nitrogen-starvation-induced autophagy in  S. cerevisiae (Tanida,  et al., 1999  ), as well as  CVT2, a gene necessary for constitutive delivery of pro-API from the cytosol to the vacuole by autophagy in  S. cerevisiae (Kim,  et al., 1999  ).	gene_phenotype
68202	3	333248	7	NULL	NULL	0	NULL	APG7	GP		is required for					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_10_5_1353_s_228	10233149	YHR171w has recently been characterized and identified as  APG7, a gene required for nitrogen-starvation-induced autophagy in  S. cerevisiae (Tanida,  et al., 1999  ), as well as  CVT2, a gene necessary for constitutive delivery of pro-API from the cytosol to the vacuole by autophagy in  S. cerevisiae (Kim,  et al., 1999  ).	gene_phenotype
68203	4	333248	7	NULL	NULL	NULL	NULL	pro-API	GP		 delivered from		constitutively			cytosol	CellComponent				NULL	S.cerevisiae	NULL	NULL	NULL	NULL	gw60_molbiolcell_10_5_1353_s_228	10233149	YHR171w has recently been characterized and identified as  APG7, a gene required for nitrogen-starvation-induced autophagy in  S. cerevisiae (Tanida,  et al., 1999  ), as well as  CVT2, a gene necessary for constitutive delivery of pro-API from the cytosol to the vacuole by autophagy in  S. cerevisiae (Kim,  et al., 1999  ).	gene_phenotype
68204	5	333248	7	NULL	NULL	NULL	NULL	pro-API	GP		 delivered to		constitutively			vacuole	CellComponent				NULL	S.cerevisiae	NULL	NULL	NULL	NULL	gw60_molbiolcell_10_5_1353_s_228	10233149	YHR171w has recently been characterized and identified as  APG7, a gene required for nitrogen-starvation-induced autophagy in  S. cerevisiae (Tanida,  et al., 1999  ), as well as  CVT2, a gene necessary for constitutive delivery of pro-API from the cytosol to the vacuole by autophagy in  S. cerevisiae (Kim,  et al., 1999  ).	gene_phenotype
68205	6	333248	7	NULL	NULL	0	NULL	statement 4	Process		occur along with					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_10_5_1353_s_228	10233149	YHR171w has recently been characterized and identified as  APG7, a gene required for nitrogen-starvation-induced autophagy in  S. cerevisiae (Tanida,  et al., 1999  ), as well as  CVT2, a gene necessary for constitutive delivery of pro-API from the cytosol to the vacuole by autophagy in  S. cerevisiae (Kim,  et al., 1999  ).	gene_phenotype
68206	7	333248	7	NULL	NULL	0	NULL	statement 6	Process		occur by					autophagy	Process				NULL	S.cerevisiae	0	NULL	NULL	NULL	gw60_molbiolcell_10_5_1353_s_228	10233149	YHR171w has recently been characterized and identified as  APG7, a gene required for nitrogen-starvation-induced autophagy in  S. cerevisiae (Tanida,  et al., 1999  ), as well as  CVT2, a gene necessary for constitutive delivery of pro-API from the cytosol to the vacuole by autophagy in  S. cerevisiae (Kim,  et al., 1999  ).	gene_phenotype
68207	8	333248	7	NULL	NULL	0	NULL	CVT2	GP		is necessary for					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_10_5_1353_s_228	10233149	YHR171w has recently been characterized and identified as  APG7, a gene required for nitrogen-starvation-induced autophagy in  S. cerevisiae (Tanida,  et al., 1999  ), as well as  CVT2, a gene necessary for constitutive delivery of pro-API from the cytosol to the vacuole by autophagy in  S. cerevisiae (Kim,  et al., 1999  ).	gene_phenotype
68208	1	333251	7	NULL	NULL	0	NULL	PDR15	GP		is a type of					major facilitator superfamily transporter	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_13_11427_s_6	12529331	These target genes code for ATP-binding cassette or major facilitator superfamily transporters such as  PDR15,  YOR1, or  AZR1 or for other proteins such as  SNG1,  YJL216c, or  YLL056c which are already known to be involved in the yeast pleiotropic drug resistance (PDR) phenomenon.	gene_phenotype
68209	2	333251	7	NULL	NULL	0	NULL	YOR1	GP		is a type of					major facilitator superfamily transporter	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_13_11427_s_6	12529331	These target genes code for ATP-binding cassette or major facilitator superfamily transporters such as  PDR15,  YOR1, or  AZR1 or for other proteins such as  SNG1,  YJL216c, or  YLL056c which are already known to be involved in the yeast pleiotropic drug resistance (PDR) phenomenon.	gene_phenotype
68210	3	333251	7	NULL	NULL	0	NULL	AZR1	GP		is a type of					major facilitator superfamily transporter	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_13_11427_s_6	12529331	These target genes code for ATP-binding cassette or major facilitator superfamily transporters such as  PDR15,  YOR1, or  AZR1 or for other proteins such as  SNG1,  YJL216c, or  YLL056c which are already known to be involved in the yeast pleiotropic drug resistance (PDR) phenomenon.	gene_phenotype
68211	4	333251	7	NULL	NULL	0	NULL	SNG1	GP		is involved in					PDR phenomenon	Process	yeast			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_13_11427_s_6	12529331	These target genes code for ATP-binding cassette or major facilitator superfamily transporters such as  PDR15,  YOR1, or  AZR1 or for other proteins such as  SNG1,  YJL216c, or  YLL056c which are already known to be involved in the yeast pleiotropic drug resistance (PDR) phenomenon.	gene_phenotype
68212	5	333251	7	NULL	NULL	0	NULL	YJL216c	GP		is involved in					PDR phenomenon	Process	yeast			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_13_11427_s_6	12529331	These target genes code for ATP-binding cassette or major facilitator superfamily transporters such as  PDR15,  YOR1, or  AZR1 or for other proteins such as  SNG1,  YJL216c, or  YLL056c which are already known to be involved in the yeast pleiotropic drug resistance (PDR) phenomenon.	gene_phenotype
68213	6	333251	7	NULL	NULL	0	NULL	YLL056c 	GP		is involved in					PDR phenomenon	Process	yeast			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_13_11427_s_6	12529331	These target genes code for ATP-binding cassette or major facilitator superfamily transporters such as  PDR15,  YOR1, or  AZR1 or for other proteins such as  SNG1,  YJL216c, or  YLL056c which are already known to be involved in the yeast pleiotropic drug resistance (PDR) phenomenon.	gene_phenotype
68214	7	333251	7	NULL	NULL	0	NULL	PDR	Process		is					pleiotropic drug resistance	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_13_11427_s_6	12529331	These target genes code for ATP-binding cassette or major facilitator superfamily transporters such as  PDR15,  YOR1, or  AZR1 or for other proteins such as  SNG1,  YJL216c, or  YLL056c which are already known to be involved in the yeast pleiotropic drug resistance (PDR) phenomenon.	gene_phenotype
68215	1	333252	7	NULL	NULL	NULL	NULL	TORC1	GP		controls			subunit of		growth	Process				NULL		NULL	NULL	NULL	NULL	gw70_yeast_23_3_159_s_74	16498703	YJR066w, YKL203c  TOR1, TOR2 PIK-related protein kinase and rapamycin target; subunit of TORC1, a complex that  controls growth in response to nutrients by regulating translation, transcription,  ribosome biogenesis, nutrient transport and autophagy; involved in meiosis  [ 3	gene_phenotype
68216	2	333252	7	NULL	NULL	NULL	NULL	statement 1	Process		in response to					nutrients	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_yeast_23_3_159_s_74	16498703	YJR066w, YKL203c  TOR1, TOR2 PIK-related protein kinase and rapamycin target; subunit of TORC1, a complex that  controls growth in response to nutrients by regulating translation, transcription,  ribosome biogenesis, nutrient transport and autophagy; involved in meiosis  [ 3	gene_phenotype
68217	3	333252	7	NULL	NULL	0	NULL	statement 1	Process		occur by					translation	Process	regulating			NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_74	16498703	YJR066w, YKL203c  TOR1, TOR2 PIK-related protein kinase and rapamycin target; subunit of TORC1, a complex that  controls growth in response to nutrients by regulating translation, transcription,  ribosome biogenesis, nutrient transport and autophagy; involved in meiosis  [ 3	gene_phenotype
68218	4	333252	7	NULL	NULL	0	NULL	statement 1	Process		occur by					transcription	Process	regulating			NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_74	16498703	YJR066w, YKL203c  TOR1, TOR2 PIK-related protein kinase and rapamycin target; subunit of TORC1, a complex that  controls growth in response to nutrients by regulating translation, transcription,  ribosome biogenesis, nutrient transport and autophagy; involved in meiosis  [ 3	gene_phenotype
68219	5	333252	7	NULL	NULL	0	NULL	statement 1	Process		occur by					ribosome biogenesis	Process	regulating			NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_74	16498703	YJR066w, YKL203c  TOR1, TOR2 PIK-related protein kinase and rapamycin target; subunit of TORC1, a complex that  controls growth in response to nutrients by regulating translation, transcription,  ribosome biogenesis, nutrient transport and autophagy; involved in meiosis  [ 3	gene_phenotype
68220	6	333252	7	NULL	NULL	0	NULL	statement 1	Process		occur by					nutrient transport 	Process	regulating			NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_74	16498703	YJR066w, YKL203c  TOR1, TOR2 PIK-related protein kinase and rapamycin target; subunit of TORC1, a complex that  controls growth in response to nutrients by regulating translation, transcription,  ribosome biogenesis, nutrient transport and autophagy; involved in meiosis  [ 3	gene_phenotype
68221	7	333252	7	NULL	NULL	0	NULL	statement 1	Process		occur by					autophagy	Process	regulating			NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_74	16498703	YJR066w, YKL203c  TOR1, TOR2 PIK-related protein kinase and rapamycin target; subunit of TORC1, a complex that  controls growth in response to nutrients by regulating translation, transcription,  ribosome biogenesis, nutrient transport and autophagy; involved in meiosis  [ 3	gene_phenotype
68222	8	333252	7	NULL	NULL	0	NULL	TORC1	GP		is involved in			subunit of		meiosis	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_74	16498703	YJR066w, YKL203c  TOR1, TOR2 PIK-related protein kinase and rapamycin target; subunit of TORC1, a complex that  controls growth in response to nutrients by regulating translation, transcription,  ribosome biogenesis, nutrient transport and autophagy; involved in meiosis  [ 3	gene_phenotype
68223	1	333253	7	NULL	NULL	0	NULL	Srx1	GP	yeast	is present in					cytosol	CellComponent				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_49_50994_s_229	15448164	Although a global analysis of protein localization in budding yeast showed that yeast Srx (Srx1, YKL086W) was present in both cytosol and the nucleus ( ) ( yeastgfp.	gene_phenotype
68224	2	333253	7	NULL	NULL	0	NULL	Srx1	GP	yeast	is present in					nucleus	CellComponent				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_49_50994_s_229	15448164	Although a global analysis of protein localization in budding yeast showed that yeast Srx (Srx1, YKL086W) was present in both cytosol and the nucleus ( ) ( yeastgfp.	gene_phenotype
68225	3	333253	7	NULL	NULL	NULL	NULL	YKL086W	GP	yeast	is present in					cytosol	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_49_50994_s_229	15448164	Although a global analysis of protein localization in budding yeast showed that yeast Srx (Srx1, YKL086W) was present in both cytosol and the nucleus ( ) ( yeastgfp.	gene_phenotype
68226	4	333253	7	NULL	NULL	0	NULL	YKL086W	GP	yeast	is present in					nucleus	CellComponent				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_49_50994_s_229	15448164	Although a global analysis of protein localization in budding yeast showed that yeast Srx (Srx1, YKL086W) was present in both cytosol and the nucleus ( ) ( yeastgfp.	gene_phenotype
68227	1	333254	7	NULL	NULL	0	NULL	YPT52 YKR014C Rab5-like GTPase	GP		is involved in					vacuolar protein 	GP	sorting of			NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_359	15334557	YPT52   YKR014C Rab5-like GTPase involved in vacuolar protein sorting and endocytosis	gene_phenotype
68228	2	333254	7	NULL	NULL	0	NULL	YPT52 YKR014C Rab5-like GTPase	GP		is involved in					endocytosis	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_359	15334557	YPT52   YKR014C Rab5-like GTPase involved in vacuolar protein sorting and endocytosis	gene_phenotype
68229	1	333255	7	NULL	NULL	0	NULL	Gog5	GP	S. cerevisiae	is a type of					vanadate resistance protein	GP	S. cerevisiae			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1593_2_179_s_296	12581862	The sponge large subunit shares with the  S. cerevisiae vanadate resistance protein Gog5 (Z46659) an  E value of only 1.6; with respect to the small subunit, the  E value to the yeast cell viability protein Ylr409cp (U19729) is even only 2.4, as  estimated in the database [ 31].	gene_phenotype
68230	2	333255	7	NULL	NULL	0	NULL	Ylr409cp	GP		is a type of					yeast cell viability protein	GP				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1593_2_179_s_296	12581862	The sponge large subunit shares with the  S. cerevisiae vanadate resistance protein Gog5 (Z46659) an  E value of only 1.6; with respect to the small subunit, the  E value to the yeast cell viability protein Ylr409cp (U19729) is even only 2.4, as  estimated in the database [ 31].	gene_phenotype
68231	1	333258	7	NULL	NULL	0	NULL	Ylr453c Rif2 2 Protein	GP		bind					Rap1p	GP		C-terminus		NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_150	16498703	Ylr453c  Rif2  2 Protein that binds to the Rap1p C-terminus and acts synergistically with Rif1p to  help control telomere length and establish telomeric silencing; deletion results  in telomere elongation  L2H  [ 24]	gene_phenotype
68232	2	333258	7	NULL	NULL	0	NULL	Ylr453c Rif2 2 Protein	GP		act synergistically with					Rif1p	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_150	16498703	Ylr453c  Rif2  2 Protein that binds to the Rap1p C-terminus and acts synergistically with Rif1p to  help control telomere length and establish telomeric silencing; deletion results  in telomere elongation  L2H  [ 24]	gene_phenotype
68233	3	333258	7	NULL	NULL	NULL	NULL	statement 2	Process		help to					telomere length	Chromosome	control			NULL		NULL	NULL	NULL	NULL	gw70_yeast_23_3_159_s_150	16498703	Ylr453c  Rif2  2 Protein that binds to the Rap1p C-terminus and acts synergistically with Rif1p to  help control telomere length and establish telomeric silencing; deletion results  in telomere elongation  L2H  [ 24]	gene_phenotype
68234	4	333258	7	NULL	NULL	0	NULL	statement 2	Process		establish					telomeric silencing	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_150	16498703	Ylr453c  Rif2  2 Protein that binds to the Rap1p C-terminus and acts synergistically with Rif1p to  help control telomere length and establish telomeric silencing; deletion results  in telomere elongation  L2H  [ 24]	gene_phenotype
68235	5	333258	7	NULL	NULL	0	NULL	statement 2	Process	deletion of	results in					telomere elongation L2H	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_150	16498703	Ylr453c  Rif2  2 Protein that binds to the Rap1p C-terminus and acts synergistically with Rif1p to  help control telomere length and establish telomeric silencing; deletion results  in telomere elongation  L2H  [ 24]	gene_phenotype
68236	1	333262	7	NULL	NULL	0	NULL	Ypl032c Svl3 1 Protein	GP	mutant;;phenotype of	suggests					 vacuolar function	Process	potential role in			NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_137	16498703	Ypl032c  Svl3  1 Protein of unknown function, mutant phenotype suggests a potential role in vacuolar  function; green fluorescent protein fusion protein localizes to the cell periphery,  cytoplasm, bud and bud neck  LIP  [ 11],[ 20]	gene_phenotype
68237	1	333263	7	NULL	NULL	0	NULL	soluble vacuolar hydrolases	GP	precursors for	is transported from					late endosome	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_258	15334557	VPS28   YPL065w Protein involved in transport of precursors for soluble vacuolar hydrolases from the  late endosome to the vacuole	gene_phenotype
68238	2	333263	7	NULL	NULL	0	NULL	soluble vacuolar hydrolases	GP	precursors for	is transported to					vacuole	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_258	15334557	VPS28   YPL065w Protein involved in transport of precursors for soluble vacuolar hydrolases from the  late endosome to the vacuole	gene_phenotype
68239	3	333263	7	NULL	NULL	0	NULL	statement 1	Process		occur along with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_258	15334557	VPS28   YPL065w Protein involved in transport of precursors for soluble vacuolar hydrolases from the  late endosome to the vacuole	gene_phenotype
68240	4	333263	7	NULL	NULL	0	NULL	VPS28 YPL065w Protein	GP		is involved in					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_258	15334557	VPS28   YPL065w Protein involved in transport of precursors for soluble vacuolar hydrolases from the  late endosome to the vacuole	gene_phenotype
68241	1	333264	7	NULL	NULL	0	NULL	Cys4p	GP	activity of	requires					 pyridoxal phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_1_836_s_200	16391125	It is worth mentioning that Cys4p requires pyridoxal phosphate for its activity, and another protein identified in our studies, YPR127w, shows similarity to the  Schizosaccharomyces pombe pyridoxal reductase, thus establishing a possible link between these two proteins.	gene_phenotype
68242	1	333265	7	NULL	NULL	0	NULL	YPR141c KAR3	GP		directs			Minus-end		microtubule motor	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_85	16498703	YPR141c   KAR3 Minus-end-directed microtubule motor that functions in mitosis and meiosis, localizes  to the spindle pole body and localization is dependent on functional Cik1p, required  for nuclear fusion during mating; potential Cdc28p substrate  [ 49]	gene_phenotype
68243	2	333265	7	NULL	NULL	0	NULL	statement 1	Process		functions in					mitosis	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_85	16498703	YPR141c   KAR3 Minus-end-directed microtubule motor that functions in mitosis and meiosis, localizes  to the spindle pole body and localization is dependent on functional Cik1p, required  for nuclear fusion during mating; potential Cdc28p substrate  [ 49]	gene_phenotype
68244	3	333265	7	NULL	NULL	0	NULL	statement 1	Process		functions in					meiosis	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_85	16498703	YPR141c   KAR3 Minus-end-directed microtubule motor that functions in mitosis and meiosis, localizes  to the spindle pole body and localization is dependent on functional Cik1p, required  for nuclear fusion during mating; potential Cdc28p substrate  [ 49]	gene_phenotype
68245	4	333265	7	NULL	NULL	0	NULL	statement 1	Process		localizes to					spindle pole body	Chromosome				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_85	16498703	YPR141c   KAR3 Minus-end-directed microtubule motor that functions in mitosis and meiosis, localizes  to the spindle pole body and localization is dependent on functional Cik1p, required  for nuclear fusion during mating; potential Cdc28p substrate  [ 49]	gene_phenotype
68246	5	333265	7	NULL	NULL	0	NULL	statement 4	Process	localization of	depends on					Cik1p	GP	functional			NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_85	16498703	YPR141c   KAR3 Minus-end-directed microtubule motor that functions in mitosis and meiosis, localizes  to the spindle pole body and localization is dependent on functional Cik1p, required  for nuclear fusion during mating; potential Cdc28p substrate  [ 49]	gene_phenotype
68247	6	333265	7	NULL	NULL	0	NULL	statement 1	Process		required for					nuclear fusion	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_85	16498703	YPR141c   KAR3 Minus-end-directed microtubule motor that functions in mitosis and meiosis, localizes  to the spindle pole body and localization is dependent on functional Cik1p, required  for nuclear fusion during mating; potential Cdc28p substrate  [ 49]	gene_phenotype
68248	7	333265	7	NULL	NULL	0	NULL	statement 6	Process		occur during					mating	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_85	16498703	YPR141c   KAR3 Minus-end-directed microtubule motor that functions in mitosis and meiosis, localizes  to the spindle pole body and localization is dependent on functional Cik1p, required  for nuclear fusion during mating; potential Cdc28p substrate  [ 49]	gene_phenotype
68249	8	333265	7	NULL	NULL	0	NULL	statement 1	Process		is substrate for					Cdc28p	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_85	16498703	YPR141c   KAR3 Minus-end-directed microtubule motor that functions in mitosis and meiosis, localizes  to the spindle pole body and localization is dependent on functional Cik1p, required  for nuclear fusion during mating; potential Cdc28p substrate  [ 49]	gene_phenotype
68270	1	333267	7	NULL	NULL	0	NULL	S. cerevisiae	Organism		encode					Rri1p	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_37_34948_s_299	11457827	This activity appears to be conserved from budding yeast to humans, even though  S. cerevisiae encodes only one COP9 signalosome subunit ortholog termed Rri1p, a Mov34 family protein previously called D0888 ( 10) or YDL216c ( 14,  15).	gene_phenotype
68271	2	333267	7	NULL	NULL	0	NULL	Rri1p	GP		is orthologous to					COP9 signalosome subunit	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_37_34948_s_299	11457827	This activity appears to be conserved from budding yeast to humans, even though  S. cerevisiae encodes only one COP9 signalosome subunit ortholog termed Rri1p, a Mov34 family protein previously called D0888 ( 10) or YDL216c ( 14,  15).	gene_phenotype
68272	3	333267	7	NULL	NULL	0	NULL	Rri1p	GP		is a type of					Mov34 family protein 	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_37_34948_s_299	11457827	This activity appears to be conserved from budding yeast to humans, even though  S. cerevisiae encodes only one COP9 signalosome subunit ortholog termed Rri1p, a Mov34 family protein previously called D0888 ( 10) or YDL216c ( 14,  15).	gene_phenotype
68274	4	333267	7	NULL	NULL	NULL	NULL	Mov34 family protein 	GP		called as		previously			D0888	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_37_34948_s_299	11457827	This activity appears to be conserved from budding yeast to humans, even though  S. cerevisiae encodes only one COP9 signalosome subunit ortholog termed Rri1p, a Mov34 family protein previously called D0888 ( 10) or YDL216c ( 14,  15).	gene_phenotype
68275	5	333267	7	NULL	NULL	NULL	NULL	Mov34 family protein 	GP		 called as		previously			YDL216c	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_37_34948_s_299	11457827	This activity appears to be conserved from budding yeast to humans, even though  S. cerevisiae encodes only one COP9 signalosome subunit ortholog termed Rri1p, a Mov34 family protein previously called D0888 ( 10) or YDL216c ( 14,  15).	gene_phenotype
68279	1	333268	7	NULL	NULL	0	NULL	AKR1 YDR264c Protein	GP	palmitoylation of	required for					pheromone receptors	GP	endocytosis of			NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_267	15334557	AKR1   YDR264c Protein palmitoylation; required for endocytosis of pheromone receptors	gene_phenotype
68297	1	333271	7	NULL	NULL	0	NULL	FYV13 YGR160w	GP		required for					yeast viability	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_309	15334557	FYV13   YGR160w Required for yeast viability on toxin exposure	gene_phenotype
68298	2	333271	7	NULL	NULL	NULL	NULL	statement 1	Process		occur upon					toxin	GP	exposure to			NULL		NULL	NULL	NULL	NULL	gw70_yeast_21_11_927_s_309	15334557	FYV13   YGR160w Required for yeast viability on toxin exposure	gene_phenotype
68299	1	333272	7	NULL	NULL	0	NULL	YHR187W	GP		recovered from					 K. lactis toxin	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_32_29628_s_60	11390369	YHR187W was previously recovered from a genetic screen for resistance to killing by  K. lactis toxin ( 11) and named  IKI1.	gene_phenotype
68300	2	333272	7	NULL	NULL	0	NULL	 K. lactis toxin	GP		is					IKI1	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_32_29628_s_60	11390369	YHR187W was previously recovered from a genetic screen for resistance to killing by  K. lactis toxin ( 11) and named  IKI1.	gene_phenotype
68301	1	333273	7	NULL	NULL	0	NULL	cAMP-dependent protein kinase	GP	cytoplasmic	contains			YJL164c TPK1 Subunit of					Tpk1p		NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_76	16498703	YJL164c   TPK1 Subunit of cytoplasmic cAMP-dependent protein kinase, which contains redundant catalytic  subunits Tpk1p, Tpk2p, and Tpk3p and regulatory subunit Bcy1p; promotes vegetative  growth in response to nutrients; inhibits filamentous growth  [ 18]	gene_phenotype
68302	2	333273	7	NULL	NULL	0	NULL	cAMP-dependent protein kinase	GP	cytoplasmic	contains			YJL164c TPK1 Subunit of					Tpk2p		NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_76	16498703	YJL164c   TPK1 Subunit of cytoplasmic cAMP-dependent protein kinase, which contains redundant catalytic  subunits Tpk1p, Tpk2p, and Tpk3p and regulatory subunit Bcy1p; promotes vegetative  growth in response to nutrients; inhibits filamentous growth  [ 18]	gene_phenotype
68303	3	333273	7	NULL	NULL	0	NULL	cAMP-dependent protein kinase	GP	cytoplasmic	contains			YJL164c TPK1 Subunit of					Tpk3p		NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_76	16498703	YJL164c   TPK1 Subunit of cytoplasmic cAMP-dependent protein kinase, which contains redundant catalytic  subunits Tpk1p, Tpk2p, and Tpk3p and regulatory subunit Bcy1p; promotes vegetative  growth in response to nutrients; inhibits filamentous growth  [ 18]	gene_phenotype
68304	4	333273	7	NULL	NULL	0	NULL	cAMP-dependent protein kinase	GP	cytoplasmic	contains			YJL164c TPK1 Subunit of					Bcy1p		NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_76	16498703	YJL164c   TPK1 Subunit of cytoplasmic cAMP-dependent protein kinase, which contains redundant catalytic  subunits Tpk1p, Tpk2p, and Tpk3p and regulatory subunit Bcy1p; promotes vegetative  growth in response to nutrients; inhibits filamentous growth  [ 18]	gene_phenotype
68305	5	333273	7	NULL	NULL	NULL	NULL	Tpk1p	GP		is a type of					catalytic subunit	GP				NULL		NULL	NULL	NULL	NULL	gw70_yeast_23_3_159_s_76	16498703	YJL164c   TPK1 Subunit of cytoplasmic cAMP-dependent protein kinase, which contains redundant catalytic  subunits Tpk1p, Tpk2p, and Tpk3p and regulatory subunit Bcy1p; promotes vegetative  growth in response to nutrients; inhibits filamentous growth  [ 18]	gene_phenotype
68306	6	333273	7	NULL	NULL	0	NULL	Tpk2p	GP		is a type of					catalytic subunit	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_76	16498703	YJL164c   TPK1 Subunit of cytoplasmic cAMP-dependent protein kinase, which contains redundant catalytic  subunits Tpk1p, Tpk2p, and Tpk3p and regulatory subunit Bcy1p; promotes vegetative  growth in response to nutrients; inhibits filamentous growth  [ 18]	gene_phenotype
68307	7	333273	7	NULL	NULL	0	NULL	Tpk3p	GP		is a type of					catalytic subunit	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_76	16498703	YJL164c   TPK1 Subunit of cytoplasmic cAMP-dependent protein kinase, which contains redundant catalytic  subunits Tpk1p, Tpk2p, and Tpk3p and regulatory subunit Bcy1p; promotes vegetative  growth in response to nutrients; inhibits filamentous growth  [ 18]	gene_phenotype
68308	8	333273	7	NULL	NULL	0	NULL	Bcy1p	GP		is a type of					regulatory subunit	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_76	16498703	YJL164c   TPK1 Subunit of cytoplasmic cAMP-dependent protein kinase, which contains redundant catalytic  subunits Tpk1p, Tpk2p, and Tpk3p and regulatory subunit Bcy1p; promotes vegetative  growth in response to nutrients; inhibits filamentous growth  [ 18]	gene_phenotype
68309	9	333273	7	NULL	NULL	0	NULL	cAMP-dependent protein kinase	GP	cytoplasmic	promotes			YJL164c TPK1 Subunit of 		vegetative growth	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_76	16498703	YJL164c   TPK1 Subunit of cytoplasmic cAMP-dependent protein kinase, which contains redundant catalytic  subunits Tpk1p, Tpk2p, and Tpk3p and regulatory subunit Bcy1p; promotes vegetative  growth in response to nutrients; inhibits filamentous growth  [ 18]	gene_phenotype
68310	10	333273	7	NULL	NULL	0	NULL	statement 9	Process		in response to					nutrients	Chemical				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_76	16498703	YJL164c   TPK1 Subunit of cytoplasmic cAMP-dependent protein kinase, which contains redundant catalytic  subunits Tpk1p, Tpk2p, and Tpk3p and regulatory subunit Bcy1p; promotes vegetative  growth in response to nutrients; inhibits filamentous growth  [ 18]	gene_phenotype
68311	11	333273	7	NULL	NULL	0	NULL	cAMP-dependent protein kinase	GP	cytoplasmic	inhibits			YJL164c TPK1 Subunit of		filamentous growth	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_76	16498703	YJL164c   TPK1 Subunit of cytoplasmic cAMP-dependent protein kinase, which contains redundant catalytic  subunits Tpk1p, Tpk2p, and Tpk3p and regulatory subunit Bcy1p; promotes vegetative  growth in response to nutrients; inhibits filamentous growth  [ 18]	gene_phenotype
68312	1	333275	7	NULL	NULL	0	NULL	 VPS2	GP		allelic to					DID4	GP				NULL		0	NULL	NULL	NULL	gw60_devcell_3_2_271_s_41	12194857	These studies led to the identification and cloning of two additional class E  VPS genes,  VPS2 (allelic to  DID4,  GRD7, and  REN1; SGD ORF YKL002W, hereafter referred to as  VPS2) and  VPS20 (SGD ORF YMR077C), a gene found to be required for transport of the plasma membrane protein Ste6 to the vacuole  (Kranz et al., 2001  ).	gene_phenotype
68313	2	333275	7	NULL	NULL	0	NULL	VPS2	GP		allelic to					GRD7	GP				NULL		0	NULL	NULL	NULL	gw60_devcell_3_2_271_s_41	12194857	These studies led to the identification and cloning of two additional class E  VPS genes,  VPS2 (allelic to  DID4,  GRD7, and  REN1; SGD ORF YKL002W, hereafter referred to as  VPS2) and  VPS20 (SGD ORF YMR077C), a gene found to be required for transport of the plasma membrane protein Ste6 to the vacuole  (Kranz et al., 2001  ).	gene_phenotype
68314	3	333275	7	NULL	NULL	0	NULL	VPS2 	GP		allelic to					REN1	GP				NULL		0	NULL	NULL	NULL	gw60_devcell_3_2_271_s_41	12194857	These studies led to the identification and cloning of two additional class E  VPS genes,  VPS2 (allelic to  DID4,  GRD7, and  REN1; SGD ORF YKL002W, hereafter referred to as  VPS2) and  VPS20 (SGD ORF YMR077C), a gene found to be required for transport of the plasma membrane protein Ste6 to the vacuole  (Kranz et al., 2001  ).	gene_phenotype
68315	4	333275	7	NULL	NULL	0	NULL	SGD ORF YKL002W	GP		is					VPS2	GP				NULL		0	NULL	NULL	NULL	gw60_devcell_3_2_271_s_41	12194857	These studies led to the identification and cloning of two additional class E  VPS genes,  VPS2 (allelic to  DID4,  GRD7, and  REN1; SGD ORF YKL002W, hereafter referred to as  VPS2) and  VPS20 (SGD ORF YMR077C), a gene found to be required for transport of the plasma membrane protein Ste6 to the vacuole  (Kranz et al., 2001  ).	gene_phenotype
68316	5	333275	7	NULL	NULL	0	NULL	VPS20	GP		is					SGD ORF YMR077C	GP				NULL		0	NULL	NULL	NULL	gw60_devcell_3_2_271_s_41	12194857	These studies led to the identification and cloning of two additional class E  VPS genes,  VPS2 (allelic to  DID4,  GRD7, and  REN1; SGD ORF YKL002W, hereafter referred to as  VPS2) and  VPS20 (SGD ORF YMR077C), a gene found to be required for transport of the plasma membrane protein Ste6 to the vacuole  (Kranz et al., 2001  ).	gene_phenotype
68317	6	333275	7	NULL	NULL	0	NULL	Ste6	GP		transported to					vacuole	CellComponent				NULL		0	NULL	NULL	NULL	gw60_devcell_3_2_271_s_41	12194857	These studies led to the identification and cloning of two additional class E  VPS genes,  VPS2 (allelic to  DID4,  GRD7, and  REN1; SGD ORF YKL002W, hereafter referred to as  VPS2) and  VPS20 (SGD ORF YMR077C), a gene found to be required for transport of the plasma membrane protein Ste6 to the vacuole  (Kranz et al., 2001  ).	gene_phenotype
68318	7	333275	7	NULL	NULL	0	NULL	Ste6	GP		is a type of					plasma membrane protein	GP				NULL		0	NULL	NULL	NULL	gw60_devcell_3_2_271_s_41	12194857	These studies led to the identification and cloning of two additional class E  VPS genes,  VPS2 (allelic to  DID4,  GRD7, and  REN1; SGD ORF YKL002W, hereafter referred to as  VPS2) and  VPS20 (SGD ORF YMR077C), a gene found to be required for transport of the plasma membrane protein Ste6 to the vacuole  (Kranz et al., 2001  ).	gene_phenotype
68319	8	333275	7	NULL	NULL	0	NULL	VPS20	GP		is required for					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_devcell_3_2_271_s_41	12194857	These studies led to the identification and cloning of two additional class E  VPS genes,  VPS2 (allelic to  DID4,  GRD7, and  REN1; SGD ORF YKL002W, hereafter referred to as  VPS2) and  VPS20 (SGD ORF YMR077C), a gene found to be required for transport of the plasma membrane protein Ste6 to the vacuole  (Kranz et al., 2001  ).	gene_phenotype
68320	1	333276	7	NULL	NULL	0	NULL	Ylr435wp	GP		is					Tsr2	GP				NULL		0	NULL	NULL	NULL	gw60_cell_113_7_919_s_161	12837249	The second protein, Ylr435wp (referred to hereafter as Tsr2, for  Twenty  S RNA accumulation), is nonessential, but deletion resulted in slow growth (doubling time  2.5 hr) in addition to a prominent 20S accumulation and a corresponding 18S deficit   (Figure 4B).	gene_phenotype
68321	2	333276	7	NULL	NULL	0	NULL	Ylr435wp	GP	deletion of	results in					slow growth	Process				NULL		0	NULL	NULL	NULL	gw60_cell_113_7_919_s_161	12837249	The second protein, Ylr435wp (referred to hereafter as Tsr2, for  Twenty  S RNA accumulation), is nonessential, but deletion resulted in slow growth (doubling time  2.5 hr) in addition to a prominent 20S accumulation and a corresponding 18S deficit   (Figure 4B).	gene_phenotype
68322	1	333279	7	NULL	NULL	0	NULL	YNL310c	GP		encode					Zim17	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_50243_s_121	15383543	Zim17 Is an Essential Component of the Import Machinery --  YNL310c, the gene encoding Zim17, is essential for viability (data not shown) ( ).	gene_phenotype
68323	2	333279	7	NULL	NULL	0	NULL	Zim17	GP		is essential for					viability	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_50243_s_121	15383543	Zim17 Is an Essential Component of the Import Machinery --  YNL310c, the gene encoding Zim17, is essential for viability (data not shown) ( ).	gene_phenotype
68324	3	333279	7	NULL	NULL	0	NULL	Zim17	GP		is essential component of					Import Machinery	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_50243_s_121	15383543	Zim17 Is an Essential Component of the Import Machinery --  YNL310c, the gene encoding Zim17, is essential for viability (data not shown) ( ).	gene_phenotype
68325	1	333280	7	NULL	NULL	0	NULL	YNL310c plasmid	NucleicAcid		maintains					cell viability	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_50243_s_152	15383543	A plasmid with YNL310c under constitutive control maintains cell viability and the cells ( Zim17) remain viable and divide to form large colonies.	gene_phenotype
68326	2	333280	7	NULL	NULL	0	NULL	statement 1	Process		under					constitutive control	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_50243_s_152	15383543	A plasmid with YNL310c under constitutive control maintains cell viability and the cells ( Zim17) remain viable and divide to form large colonies.	gene_phenotype
68327	1	333281	7	NULL	NULL	NULL	NULL	 yTRN	GP		interact with					M9-containing import substrates	GP	members of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_4141_s_219	9632798	It seems that yTRN is more constrained than hTRN1 in its capacity to interact with various members of the M9-containing import substrates, although yTRN does apparently bind Nab4p (YOL123w or Hrp1p) ( 2), another nuclear mRNA-binding protein in  S. cerevisiae.	gene_phenotype
68328	2	333281	7	NULL	NULL	NULL	NULL	hTRN1 	GP		interact with					M9-containing import substrates	GP	members of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_7_4141_s_219	9632798	It seems that yTRN is more constrained than hTRN1 in its capacity to interact with various members of the M9-containing import substrates, although yTRN does apparently bind Nab4p (YOL123w or Hrp1p) ( 2), another nuclear mRNA-binding protein in  S. cerevisiae.	gene_phenotype
68329	3	333281	7	NULL	NULL	0	NULL	statement 1	Process		is more constrained than					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_7_4141_s_219	9632798	It seems that yTRN is more constrained than hTRN1 in its capacity to interact with various members of the M9-containing import substrates, although yTRN does apparently bind Nab4p (YOL123w or Hrp1p) ( 2), another nuclear mRNA-binding protein in  S. cerevisiae.	gene_phenotype
68330	4	333281	7	NULL	NULL	0	NULL	yTRN	GP		bind					Nab4p	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_7_4141_s_219	9632798	It seems that yTRN is more constrained than hTRN1 in its capacity to interact with various members of the M9-containing import substrates, although yTRN does apparently bind Nab4p (YOL123w or Hrp1p) ( 2), another nuclear mRNA-binding protein in  S. cerevisiae.	gene_phenotype
68331	5	333281	7	NULL	NULL	0	NULL	Nab4p 	GP		is a type of					nuclear mRNA-binding protein					NULL	S.cerevisiae	0	NULL	NULL	NULL	gw60_molcellbiol_18_7_4141_s_219	9632798	It seems that yTRN is more constrained than hTRN1 in its capacity to interact with various members of the M9-containing import substrates, although yTRN does apparently bind Nab4p (YOL123w or Hrp1p) ( 2), another nuclear mRNA-binding protein in  S. cerevisiae.	gene_phenotype
68332	1	333282	7	NULL	NULL	0	NULL	ODC1	GP		encode					mitochondrial transporter family	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1459_2_363_s_118	11004452	ODC1 and ODC2 (genome designation YPL134c and YOR222w, respectively) encode two closely related members of the mitochondrial transporter family (61% identity; 88% similarity).	gene_phenotype
68333	2	333282	7	NULL	NULL	0	NULL	ODC2	GP		encode					mitochondrial transporter family	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1459_2_363_s_118	11004452	ODC1 and ODC2 (genome designation YPL134c and YOR222w, respectively) encode two closely related members of the mitochondrial transporter family (61% identity; 88% similarity).	gene_phenotype
68334	1	333285	7	NULL	NULL	0	NULL	ALD5	GP		encode					NAD(P) ACDH	GP	minor form of mitochondrial			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_66_8_3151_s_53	10919763	ALD5 (YER073w) was shown to encode a minor form of the mitochondrial NAD(P) ACDH ( 49), which might play a role in regulation or biosynthesis of electron transport chain components ( 19).	gene_phenotype
68335	2	333285	7	NULL	NULL	0	NULL	NAD(P) ACDH	GP		play a role in					electron transport chain components	GP	regulation of			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_66_8_3151_s_53	10919763	ALD5 (YER073w) was shown to encode a minor form of the mitochondrial NAD(P) ACDH ( 49), which might play a role in regulation or biosynthesis of electron transport chain components ( 19).	gene_phenotype
68336	3	333285	7	NULL	NULL	0	NULL	NAD(P) ACDH	GP		play a role in					electron transport chain components	GP	biosynthesis of			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_66_8_3151_s_53	10919763	ALD5 (YER073w) was shown to encode a minor form of the mitochondrial NAD(P) ACDH ( 49), which might play a role in regulation or biosynthesis of electron transport chain components ( 19).	gene_phenotype
68337	1	333286	7	NULL	NULL	0	NULL	Pho87	GP		is a type of					putative phosphate transporter	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_12_4309_s_172	11102525	Furthermore, this similarity is shared among a total of nine  S. cerevisiae ORFs, including the putative phosphate transporter Pho87 (Bun-ya  et al., 1996  ), two proteins homologous to Pho87, Yjl198w and Ynr013, and Syg1 (Spain  et al., 1995  ), a multi-copy suppressor for a  GPA1 deletion.	gene_phenotype
68338	1	333287	7	NULL	NULL	0	NULL	ORF YJL204c	GP	strain disrupted for	shows					LY	Chemical	decreased levels of			NULL	vacuole	0	NULL	NULL	NULL	gw60_cellbiol_149_2_397_s_153	10769031	The strain, disrupted for the ORF  YJL204c, showed decreased levels of LY in the vacuole consistent with a defect in fluid-phase endocytosis (compare   Fig 1 A and   Fig 1 B).	gene_phenotype
68339	2	333287	7	NULL	NULL	0	NULL	statement 1	Process		consistent with					fluid-phase endocytosis	Process	defect in			NULL		0	NULL	NULL	NULL	gw60_cellbiol_149_2_397_s_153	10769031	The strain, disrupted for the ORF  YJL204c, showed decreased levels of LY in the vacuole consistent with a defect in fluid-phase endocytosis (compare   Fig 1 A and   Fig 1 B).	gene_phenotype
68340	1	333288	7	NULL	NULL	0	NULL	YKL146wp	GP		encode					AVT3 	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_25_22966_s_36	11959859	Recently it was shown that YKL146wp indeed codes for a protein that represents a vesicular amino acid transporter, designated as AVT3 ( 4).	gene_phenotype
68341	2	333288	7	NULL	NULL	NULL	NULL	AVT3	GP		is a type of					vesicular amino acid transporter	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_25_22966_s_36	11959859	Recently it was shown that YKL146wp indeed codes for a protein that represents a vesicular amino acid transporter, designated as AVT3 ( 4).	gene_phenotype
68342	1	333289	7	NULL	NULL	0	NULL	 YKL146wp	GP	S. cerevisiae	is a type of					putative amino acid transport protein	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_25_22966_s_35	11959859	We searched for mammalian AAAP family members based on the  S. cerevisiae protein sequence YKL146wp, which had been identified by genome-scanning analysis as a putative amino acid transport protein.	gene_phenotype
68343	1	333290	7	NULL	NULL	NULL	NULL	YKR082w	GP	double mutant	is not					viable	Process				NULL		NULL	NULL	NULL	NULL	gw60_gene_233_1_141_s_132	10375630	Alternatively, it could also be that double mutants in  YKR082w along with either  YKR081c or  YKR083c are not viable.	gene_phenotype
68344	2	333290	7	NULL	NULL	0	NULL	YKR081c	GP	double mutant	is not 					viable	Process				NULL		0	NULL	NULL	NULL	gw60_gene_233_1_141_s_132	10375630	Alternatively, it could also be that double mutants in  YKR082w along with either  YKR081c or  YKR083c are not viable.	gene_phenotype
68345	3	333290	7	NULL	NULL	0	NULL	YKR083c	GP	double mutant	is not					viable	Process				NULL		0	NULL	NULL	NULL	gw60_gene_233_1_141_s_132	10375630	Alternatively, it could also be that double mutants in  YKR082w along with either  YKR081c or  YKR083c are not viable.	gene_phenotype
68346	1	333293	7	NULL	NULL	0	NULL	ERG3	GP		is resistant to					fluconazole	Chemical				NULL		0	NULL	NULL	NULL	gw60_genetics_163_4_1287_s_10	12702675	In a genome-wide screen of  4700 viable deletion strains, 13 were classified as resistant to fluconazole ( ERG3,  ERG6,  YMR102C,  YMR099C,  YPL056C,  ERG28,  OSH1,  SCS2,  CKA2,  SML1,  YBR147W,  YGR283C, and  YLR407W).	gene_phenotype
68347	2	333293	7	NULL	NULL	0	NULL	ERG6	GP		is resistant to					fluconazole	Chemical				NULL		0	NULL	NULL	NULL	gw60_genetics_163_4_1287_s_10	12702675	In a genome-wide screen of  4700 viable deletion strains, 13 were classified as resistant to fluconazole ( ERG3,  ERG6,  YMR102C,  YMR099C,  YPL056C,  ERG28,  OSH1,  SCS2,  CKA2,  SML1,  YBR147W,  YGR283C, and  YLR407W).	gene_phenotype
68348	3	333293	7	NULL	NULL	0	NULL	YMR102C	GP		is resistant to					fluconazole	Chemical				NULL		0	NULL	NULL	NULL	gw60_genetics_163_4_1287_s_10	12702675	In a genome-wide screen of  4700 viable deletion strains, 13 were classified as resistant to fluconazole ( ERG3,  ERG6,  YMR102C,  YMR099C,  YPL056C,  ERG28,  OSH1,  SCS2,  CKA2,  SML1,  YBR147W,  YGR283C, and  YLR407W).	gene_phenotype
68349	4	333293	7	NULL	NULL	0	NULL	YMR099C	GP		is resistant to					fluconazole	Chemical				NULL		0	NULL	NULL	NULL	gw60_genetics_163_4_1287_s_10	12702675	In a genome-wide screen of  4700 viable deletion strains, 13 were classified as resistant to fluconazole ( ERG3,  ERG6,  YMR102C,  YMR099C,  YPL056C,  ERG28,  OSH1,  SCS2,  CKA2,  SML1,  YBR147W,  YGR283C, and  YLR407W).	gene_phenotype
68350	5	333293	7	NULL	NULL	0	NULL	YPL056C	GP		is resistant to					fluconazole	Chemical				NULL		0	NULL	NULL	NULL	gw60_genetics_163_4_1287_s_10	12702675	In a genome-wide screen of  4700 viable deletion strains, 13 were classified as resistant to fluconazole ( ERG3,  ERG6,  YMR102C,  YMR099C,  YPL056C,  ERG28,  OSH1,  SCS2,  CKA2,  SML1,  YBR147W,  YGR283C, and  YLR407W).	gene_phenotype
68351	6	333293	7	NULL	NULL	0	NULL	ERG28	GP		is resistant to					fluconazole	Chemical				NULL		0	NULL	NULL	NULL	gw60_genetics_163_4_1287_s_10	12702675	In a genome-wide screen of  4700 viable deletion strains, 13 were classified as resistant to fluconazole ( ERG3,  ERG6,  YMR102C,  YMR099C,  YPL056C,  ERG28,  OSH1,  SCS2,  CKA2,  SML1,  YBR147W,  YGR283C, and  YLR407W).	gene_phenotype
68352	7	333293	7	NULL	NULL	0	NULL	OSH1	GP		is resistant to					fluconazole	Chemical				NULL		0	NULL	NULL	NULL	gw60_genetics_163_4_1287_s_10	12702675	In a genome-wide screen of  4700 viable deletion strains, 13 were classified as resistant to fluconazole ( ERG3,  ERG6,  YMR102C,  YMR099C,  YPL056C,  ERG28,  OSH1,  SCS2,  CKA2,  SML1,  YBR147W,  YGR283C, and  YLR407W).	gene_phenotype
68353	8	333293	7	NULL	NULL	0	NULL	SCS2	GP		is resistant to					fluconazole	Chemical				NULL		0	NULL	NULL	NULL	gw60_genetics_163_4_1287_s_10	12702675	In a genome-wide screen of  4700 viable deletion strains, 13 were classified as resistant to fluconazole ( ERG3,  ERG6,  YMR102C,  YMR099C,  YPL056C,  ERG28,  OSH1,  SCS2,  CKA2,  SML1,  YBR147W,  YGR283C, and  YLR407W).	gene_phenotype
68354	9	333293	7	NULL	NULL	0	NULL	CKA2	GP		is resistant to					fluconazole	Chemical				NULL		0	NULL	NULL	NULL	gw60_genetics_163_4_1287_s_10	12702675	In a genome-wide screen of  4700 viable deletion strains, 13 were classified as resistant to fluconazole ( ERG3,  ERG6,  YMR102C,  YMR099C,  YPL056C,  ERG28,  OSH1,  SCS2,  CKA2,  SML1,  YBR147W,  YGR283C, and  YLR407W).	gene_phenotype
68355	10	333293	7	NULL	NULL	0	NULL	SML1	GP		is resistant to					fluconazole	Chemical				NULL		0	NULL	NULL	NULL	gw60_genetics_163_4_1287_s_10	12702675	In a genome-wide screen of  4700 viable deletion strains, 13 were classified as resistant to fluconazole ( ERG3,  ERG6,  YMR102C,  YMR099C,  YPL056C,  ERG28,  OSH1,  SCS2,  CKA2,  SML1,  YBR147W,  YGR283C, and  YLR407W).	gene_phenotype
68356	11	333293	7	NULL	NULL	0	NULL	YBR147W	GP		is resistant to					fluconazole	Chemical				NULL		0	NULL	NULL	NULL	gw60_genetics_163_4_1287_s_10	12702675	In a genome-wide screen of  4700 viable deletion strains, 13 were classified as resistant to fluconazole ( ERG3,  ERG6,  YMR102C,  YMR099C,  YPL056C,  ERG28,  OSH1,  SCS2,  CKA2,  SML1,  YBR147W,  YGR283C, and  YLR407W).	gene_phenotype
68357	12	333293	7	NULL	NULL	0	NULL	YGR283C	GP		is resistant to					fluconazole	Chemical				NULL		0	NULL	NULL	NULL	gw60_genetics_163_4_1287_s_10	12702675	In a genome-wide screen of  4700 viable deletion strains, 13 were classified as resistant to fluconazole ( ERG3,  ERG6,  YMR102C,  YMR099C,  YPL056C,  ERG28,  OSH1,  SCS2,  CKA2,  SML1,  YBR147W,  YGR283C, and  YLR407W).	gene_phenotype
68358	13	333293	7	NULL	NULL	0	NULL	YLR407W	GP		is resistant to					fluconazole	Chemical				NULL		0	NULL	NULL	NULL	gw60_genetics_163_4_1287_s_10	12702675	In a genome-wide screen of  4700 viable deletion strains, 13 were classified as resistant to fluconazole ( ERG3,  ERG6,  YMR102C,  YMR099C,  YPL056C,  ERG28,  OSH1,  SCS2,  CKA2,  SML1,  YBR147W,  YGR283C, and  YLR407W).	gene_phenotype
68412	1	333297	7	NULL	NULL	0	NULL	methylglyoxal	Chemical	reducing activity of	depends on					NADPH	Chemical				NULL	Cells	0	NULL	NULL	NULL	gw70_yeast_20_6_545_s_221	12722185	NADPH-dependent methylglyoxal-reducing activity in cells containing GST fusions to  the indicated ORFs (strain 1, YOL151w; strain 2, YDR541c; strain 3, YGL039w; strain  4, YGL157w; strain 5, YNL241c).	gene_phenotype
68359	1	333298	7	NULL	NULL	0	NULL	Yol082p 	GP		is not required for					vegetative growth	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_31_29210_s_88	11382752	The null mutant of  YOL082w, which as described was viable ( 20), showed wild-type growth rate in SD medium with a doubling time of 150 min for both wild-type and  deltayol082 strains, indicating that Yol082p function is not required for vegetative growth.	gene_phenotype
68360	1	333300	7	NULL	NULL	0	NULL	PHO85 YPL031c Cyclin-dependent protein kinase	GP		is involved in					phosphate metabolism	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_317	15334557	PHO85   YPL031c Cyclin-dependent protein kinase; involved in phosphate and glycogen metabolism as  well as cell cycle progression	gene_phenotype
68361	2	333300	7	NULL	NULL	0	NULL	PHO85 YPL031c Cyclin-dependent protein kinase	GP		is involved in					glycogen metabolism	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_317	15334557	PHO85   YPL031c Cyclin-dependent protein kinase; involved in phosphate and glycogen metabolism as  well as cell cycle progression	gene_phenotype
68362	3	333300	7	NULL	NULL	0	NULL	PHO85 YPL031c Cyclin-dependent protein kinase	GP		is involved in					cell cycle progression	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_317	15334557	PHO85   YPL031c Cyclin-dependent protein kinase; involved in phosphate and glycogen metabolism as  well as cell cycle progression	gene_phenotype
68363	1	333301	7	NULL	NULL	NULL	NULL	Kap95	GP		imports					NLS protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68364	2	333301	7	NULL	NULL	NULL	NULL	Kap beta1	GP		imports					NLS protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68365	3	333301	7	NULL	NULL	0	NULL	Kap alpha	GP		helps					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68366	4	333301	7	NULL	NULL	0	NULL	Kap alpha	GP		helps					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68367	5	333301	7	NULL	NULL	0	NULL	Kap alpha	GP		complex with					Kap104	GP				NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68368	6	333301	7	NULL	NULL	0	NULL	statement 5	GP		complex with					Kap beta2	GP				NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68369	7	333301	7	NULL	NULL	0	NULL	statement 6	GP		imports					PSE1, Kap121	GP				NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68370	8	333301	7	NULL	NULL	0	NULL	statement 6	GP		imports					Kap beta3	GP				NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68371	9	333301	7	NULL	NULL	0	NULL	statement 6	GP		imports					Kap123	GP				NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68372	10	333301	7	NULL	NULL	0	NULL	statement 6	GP		imports					Kap108	GP				NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68373	11	333301	7	NULL	NULL	NULL	NULL	statement 6	GP		imports					Kap111	GP				NULL		NULL	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68374	12	333301	7	NULL	NULL	0	NULL	statement 6	GP		imports					mRNA-binding proteins	GP				NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68375	13	333301	7	NULL	NULL	0	NULL	statement 6	GP		exports		possibly			mRNA-binding proteins	GP				NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68376	14	333301	7	NULL	NULL	0	NULL	CSE1 CAS	GP		exports					 karyopherin alpha	GP				NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68377	15	333301	7	NULL	NULL	0	NULL	LOS1	GP		transports		possibly			tRNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68378	16	333301	7	NULL	NULL	0	NULL	XPO1 exportin	GP		exports					PDR6	GP				NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68379	17	333301	7	NULL	NULL	0	NULL	Kap alpha	GP		is					Karyopherin alpha Importin alpha	GP				NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68380	18	333301	7	NULL	NULL	0	NULL	Kap95	GP		is					Karyopherin beta1	GP				NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68381	19	333301	7	NULL	NULL	0	NULL	Kap beta1	GP		is					 Importin beta	GP				NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68382	20	333301	7	NULL	NULL	0	NULL	Kap95	GP		is a type of					import protein	GP				NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68383	21	333301	7	NULL	NULL	0	NULL	Kap beta1	GP		is a type of					import protein	GP				NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68384	22	333301	7	NULL	NULL	0	NULL	Kap104	GP		is					Karyopherin beta2	GP				NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68385	23	333301	7	NULL	NULL	0	NULL	Kap beta2	GP		is					transportin	GP				NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68386	24	333301	7	NULL	NULL	0	NULL	PSE1, Kap121	GP		is					hnRNPA1 Karyopherin beta3	GP				NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68387	25	333301	7	NULL	NULL	0	NULL	PSE1, Kap121	GP		is a type of					mRNA-binding proteins	GP				NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68388	26	333301	7	NULL	NULL	0	NULL	Kap123	GP		is					Karyopherin beta4	GP				NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68389	27	333301	7	NULL	NULL	0	NULL	Kap108	GP		is					SXM1	GP				NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68390	28	333301	7	NULL	NULL	0	NULL	Kap108	GP		is a type of					ribosomal protein	GP				NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68391	29	333301	7	NULL	NULL	0	NULL	Kap111	GP		is					MTR10	GP				NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68392	30	333301	7	NULL	NULL	0	NULL	PDR6	GP		contains					leucine-rich export sequences 	AminoAcid				NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68393	31	333301	7	NULL	NULL	0	NULL	PDR6 	GP		belongs to					karyopherin b4 family	GP				NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68396	32	333301	7	NULL	NULL	0	NULL	KAP111	GP		is involved in					tRNA	NucleicAcid	processing			NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68397	33	333301	7	NULL	NULL	0	NULL	KAp111	GP		is involved in					mRNA	NucleicAcid	processing			NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1129_s_45	9508684	THE WORLD OF NUCLEAR TRANSPORTERS  Yeast Protein Homologs Function  Karyopherin alpha Importin  alpha (Kap  alpha) Helps import proteins with NLS sequences  Karyopherin beta1 (Kap95) Importin beta (Kap beta1) Imports NLS proteins, complexed with karyopherin  alpha (importin alpha)  Karyopherin beta2  (Kap104) transportin  (Kap beta2) Imports mRNA-binding proteins, such as hnRNPA1  Karyopherin beta3 (PSE1, Kap121) Kap beta3 Imports ribosomal proteins  Karyopherin beta4 (Kap123)   Imports ribosomal proteins  *SXM1  (Kap108)   Imports proteins involved in  processing tRNA and possibly mRNA  *MTR10  (Kap111)   Imports and possibly exports  mRNA-binding proteins  *CSE1 CAS Exports karyopherin  alpha  (importin  alpha)  *NMD5 Ran BP7,  [[ Ran BP8 Unknown  *LOS1   Possibly transports tRNA  *MSN5   Unknown  *CRM1 ]], XPO1  (Kap124) Exportin Exports proteins with leucine-rich export sequences  *PDR6   [[ Unknown  *YGL241W   Unknown  *YPL125W   Unknown  * Members ]] of the karyopherin b4 family	gene_phenotype
68398	1	333302	7	NULL	NULL	0	NULL	isw2delta	GP	mutation of	enhance		slightly			telomere-silencing defect					NULL	dpb4delta mutant cells	0	NULL	NULL	NULL	gw70_molcellbiol_24_1_217_s_180	14673157	On the other hand, the  isw2delta mutation slightly enhanced the telomere-silencing defect in  dpb4delta mutant cells, suggesting that the Isw2 protein solely, not as a complex, or a putative complex of Isw2 with the other WAC domain protein ( ), such as a product from YPL216w, plays a putative positive role in TPE.	gene_phenotype
68399	2	333302	7	NULL	NULL	NULL	NULL	Isw2 protein	GP		complex with		putatively			YPL216w	GP	product of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_1_217_s_180	14673157	On the other hand, the  isw2delta mutation slightly enhanced the telomere-silencing defect in  dpb4delta mutant cells, suggesting that the Isw2 protein solely, not as a complex, or a putative complex of Isw2 with the other WAC domain protein ( ), such as a product from YPL216w, plays a putative positive role in TPE.	gene_phenotype
68400	3	333302	7	NULL	NULL	0	NULL	YPL216w	GP	product of	is a type of					WAC domain protein	GP				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_1_217_s_180	14673157	On the other hand, the  isw2delta mutation slightly enhanced the telomere-silencing defect in  dpb4delta mutant cells, suggesting that the Isw2 protein solely, not as a complex, or a putative complex of Isw2 with the other WAC domain protein ( ), such as a product from YPL216w, plays a putative positive role in TPE.	gene_phenotype
68401	4	333302	7	NULL	NULL	NULL	NULL	YPL216w	GP	product of	positive role in		putative			TPE	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_1_217_s_180	14673157	On the other hand, the  isw2delta mutation slightly enhanced the telomere-silencing defect in  dpb4delta mutant cells, suggesting that the Isw2 protein solely, not as a complex, or a putative complex of Isw2 with the other WAC domain protein ( ), such as a product from YPL216w, plays a putative positive role in TPE.	gene_phenotype
68402	5	333302	7	NULL	NULL	NULL	NULL	Isw2 protein	GP		positive role in		putative			TPE	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_1_217_s_180	14673157	On the other hand, the  isw2delta mutation slightly enhanced the telomere-silencing defect in  dpb4delta mutant cells, suggesting that the Isw2 protein solely, not as a complex, or a putative complex of Isw2 with the other WAC domain protein ( ), such as a product from YPL216w, plays a putative positive role in TPE.	gene_phenotype
68413	1	333303	7	NULL	NULL	0	NULL	 VMA11	GP		encode					 vacuolar ATPase	GP		proteolipid subunit of 		NULL		0	NULL	NULL	NULL	gw60_genetics_161_2_585_s_169	12072456	One is the unknown ORF YPL233w; two are known genes:  VMA11 encodes a proteolipid subunit of the vacuolar ATPase, an H[+]-translocating ATPase that hydrolyzes ATP to ADP and Pi, to drive protons across the vacuolar membrane into the lumen ( H IRATA et al. 1997   ), while  SSO1 encodes a syntaxin homolog (t-SNARE) involved in vesicle transport between the Golgi apparatus and the plasma membrane.	gene_phenotype
68414	2	333303	7	NULL	NULL	0	NULL	 vacuolar ATPase	GP		is a type of					H[+]-translocating ATPase	GP				NULL		0	NULL	NULL	NULL	gw60_genetics_161_2_585_s_169	12072456	One is the unknown ORF YPL233w; two are known genes:  VMA11 encodes a proteolipid subunit of the vacuolar ATPase, an H[+]-translocating ATPase that hydrolyzes ATP to ADP and Pi, to drive protons across the vacuolar membrane into the lumen ( H IRATA et al. 1997   ), while  SSO1 encodes a syntaxin homolog (t-SNARE) involved in vesicle transport between the Golgi apparatus and the plasma membrane.	gene_phenotype
68415	3	333303	7	NULL	NULL	0	NULL	ATP	Chemical		hydrolyzed to					ADP	Chemical				NULL		0	NULL	NULL	NULL	gw60_genetics_161_2_585_s_169	12072456	One is the unknown ORF YPL233w; two are known genes:  VMA11 encodes a proteolipid subunit of the vacuolar ATPase, an H[+]-translocating ATPase that hydrolyzes ATP to ADP and Pi, to drive protons across the vacuolar membrane into the lumen ( H IRATA et al. 1997   ), while  SSO1 encodes a syntaxin homolog (t-SNARE) involved in vesicle transport between the Golgi apparatus and the plasma membrane.	gene_phenotype
68416	4	333303	7	NULL	NULL	0	NULL	ATP	Chemical		hydrolyzed to					Pi	Chemical				NULL		0	NULL	NULL	NULL	gw60_genetics_161_2_585_s_169	12072456	One is the unknown ORF YPL233w; two are known genes:  VMA11 encodes a proteolipid subunit of the vacuolar ATPase, an H[+]-translocating ATPase that hydrolyzes ATP to ADP and Pi, to drive protons across the vacuolar membrane into the lumen ( H IRATA et al. 1997   ), while  SSO1 encodes a syntaxin homolog (t-SNARE) involved in vesicle transport between the Golgi apparatus and the plasma membrane.	gene_phenotype
68417	5	333303	7	NULL	NULL	0	NULL	statement 3	Process		occur along with					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_161_2_585_s_169	12072456	One is the unknown ORF YPL233w; two are known genes:  VMA11 encodes a proteolipid subunit of the vacuolar ATPase, an H[+]-translocating ATPase that hydrolyzes ATP to ADP and Pi, to drive protons across the vacuolar membrane into the lumen ( H IRATA et al. 1997   ), while  SSO1 encodes a syntaxin homolog (t-SNARE) involved in vesicle transport between the Golgi apparatus and the plasma membrane.	gene_phenotype
68418	6	333303	7	NULL	NULL	0	NULL	vacuolar ATPase	GP		catalyze					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_161_2_585_s_169	12072456	One is the unknown ORF YPL233w; two are known genes:  VMA11 encodes a proteolipid subunit of the vacuolar ATPase, an H[+]-translocating ATPase that hydrolyzes ATP to ADP and Pi, to drive protons across the vacuolar membrane into the lumen ( H IRATA et al. 1997   ), while  SSO1 encodes a syntaxin homolog (t-SNARE) involved in vesicle transport between the Golgi apparatus and the plasma membrane.	gene_phenotype
68419	7	333303	7	NULL	NULL	0	NULL	protons	Chemical		move from					vacuolar membrane	CellComponent				NULL		0	NULL	NULL	NULL	gw60_genetics_161_2_585_s_169	12072456	One is the unknown ORF YPL233w; two are known genes:  VMA11 encodes a proteolipid subunit of the vacuolar ATPase, an H[+]-translocating ATPase that hydrolyzes ATP to ADP and Pi, to drive protons across the vacuolar membrane into the lumen ( H IRATA et al. 1997   ), while  SSO1 encodes a syntaxin homolog (t-SNARE) involved in vesicle transport between the Golgi apparatus and the plasma membrane.	gene_phenotype
68420	8	333303	7	NULL	NULL	0	NULL	protons	Chemical		move to					lumen	CellComponent				NULL		0	NULL	NULL	NULL	gw60_genetics_161_2_585_s_169	12072456	One is the unknown ORF YPL233w; two are known genes:  VMA11 encodes a proteolipid subunit of the vacuolar ATPase, an H[+]-translocating ATPase that hydrolyzes ATP to ADP and Pi, to drive protons across the vacuolar membrane into the lumen ( H IRATA et al. 1997   ), while  SSO1 encodes a syntaxin homolog (t-SNARE) involved in vesicle transport between the Golgi apparatus and the plasma membrane.	gene_phenotype
68421	9	333303	7	NULL	NULL	0	NULL	statement 7	Process		occur along with					statement 8	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_161_2_585_s_169	12072456	One is the unknown ORF YPL233w; two are known genes:  VMA11 encodes a proteolipid subunit of the vacuolar ATPase, an H[+]-translocating ATPase that hydrolyzes ATP to ADP and Pi, to drive protons across the vacuolar membrane into the lumen ( H IRATA et al. 1997   ), while  SSO1 encodes a syntaxin homolog (t-SNARE) involved in vesicle transport between the Golgi apparatus and the plasma membrane.	gene_phenotype
68422	10	333303	7	NULL	NULL	0	NULL	statement 5	Process		drives					statement 9	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_161_2_585_s_169	12072456	One is the unknown ORF YPL233w; two are known genes:  VMA11 encodes a proteolipid subunit of the vacuolar ATPase, an H[+]-translocating ATPase that hydrolyzes ATP to ADP and Pi, to drive protons across the vacuolar membrane into the lumen ( H IRATA et al. 1997   ), while  SSO1 encodes a syntaxin homolog (t-SNARE) involved in vesicle transport between the Golgi apparatus and the plasma membrane.	gene_phenotype
68423	11	333303	7	NULL	NULL	0	NULL	 SSO1	GP		encode					 syntaxin homolog 	GP				NULL		0	NULL	NULL	NULL	gw60_genetics_161_2_585_s_169	12072456	One is the unknown ORF YPL233w; two are known genes:  VMA11 encodes a proteolipid subunit of the vacuolar ATPase, an H[+]-translocating ATPase that hydrolyzes ATP to ADP and Pi, to drive protons across the vacuolar membrane into the lumen ( H IRATA et al. 1997   ), while  SSO1 encodes a syntaxin homolog (t-SNARE) involved in vesicle transport between the Golgi apparatus and the plasma membrane.	gene_phenotype
68424	12	333303	7	NULL	NULL	0	NULL	 syntaxin homolog 	GP		is					t-SNARE	GP				NULL		0	NULL	NULL	NULL	gw60_genetics_161_2_585_s_169	12072456	One is the unknown ORF YPL233w; two are known genes:  VMA11 encodes a proteolipid subunit of the vacuolar ATPase, an H[+]-translocating ATPase that hydrolyzes ATP to ADP and Pi, to drive protons across the vacuolar membrane into the lumen ( H IRATA et al. 1997   ), while  SSO1 encodes a syntaxin homolog (t-SNARE) involved in vesicle transport between the Golgi apparatus and the plasma membrane.	gene_phenotype
68425	13	333303	7	NULL	NULL	0	NULL	vesicle	CellComponent		transported between					golgi apparatus	CellComponent				NULL		0	NULL	NULL	NULL	gw60_genetics_161_2_585_s_169	12072456	One is the unknown ORF YPL233w; two are known genes:  VMA11 encodes a proteolipid subunit of the vacuolar ATPase, an H[+]-translocating ATPase that hydrolyzes ATP to ADP and Pi, to drive protons across the vacuolar membrane into the lumen ( H IRATA et al. 1997   ), while  SSO1 encodes a syntaxin homolog (t-SNARE) involved in vesicle transport between the Golgi apparatus and the plasma membrane.	gene_phenotype
68426	14	333303	7	NULL	NULL	0	NULL	vesicle	CellComponent		transported between					plasma membrane	CellComponent				NULL		0	NULL	NULL	NULL	gw60_genetics_161_2_585_s_169	12072456	One is the unknown ORF YPL233w; two are known genes:  VMA11 encodes a proteolipid subunit of the vacuolar ATPase, an H[+]-translocating ATPase that hydrolyzes ATP to ADP and Pi, to drive protons across the vacuolar membrane into the lumen ( H IRATA et al. 1997   ), while  SSO1 encodes a syntaxin homolog (t-SNARE) involved in vesicle transport between the Golgi apparatus and the plasma membrane.	gene_phenotype
68427	15	333303	7	NULL	NULL	0	NULL	statement 13	Process		occur along with					statement 14	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_161_2_585_s_169	12072456	One is the unknown ORF YPL233w; two are known genes:  VMA11 encodes a proteolipid subunit of the vacuolar ATPase, an H[+]-translocating ATPase that hydrolyzes ATP to ADP and Pi, to drive protons across the vacuolar membrane into the lumen ( H IRATA et al. 1997   ), while  SSO1 encodes a syntaxin homolog (t-SNARE) involved in vesicle transport between the Golgi apparatus and the plasma membrane.	gene_phenotype
68428	16	333303	7	NULL	NULL	0	NULL	t-SNARE	GP		is involved in					statement 15	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_161_2_585_s_169	12072456	One is the unknown ORF YPL233w; two are known genes:  VMA11 encodes a proteolipid subunit of the vacuolar ATPase, an H[+]-translocating ATPase that hydrolyzes ATP to ADP and Pi, to drive protons across the vacuolar membrane into the lumen ( H IRATA et al. 1997   ), while  SSO1 encodes a syntaxin homolog (t-SNARE) involved in vesicle transport between the Golgi apparatus and the plasma membrane.	gene_phenotype
68429	1	333304	7	NULL	NULL	0	NULL	 Sps2	GP		is homologous to					Ecm33	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_20_9_781_s_165	12845604	Finally, YPL261c and Sps2 (a protein with homology to GPI protein Ecm33), which  were also identified in their screen for GPI proteins, were excluded from our GPI  protein list because their N-terminal regions are unlikely to be signal peptides  for secretion.	gene_phenotype
68430	2	333304	7	NULL	NULL	0	NULL	Ecm33	GP		is a type of					GPI protein	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_20_9_781_s_165	12845604	Finally, YPL261c and Sps2 (a protein with homology to GPI protein Ecm33), which  were also identified in their screen for GPI proteins, were excluded from our GPI  protein list because their N-terminal regions are unlikely to be signal peptides  for secretion.	gene_phenotype
68431	4	333304	7	NULL	NULL	NULL	NULL	 YPL261c	GP		does not have					signal peptides	GP		N-terminal regions		NULL		NULL	NULL	NULL	NULL	gw70_yeast_20_9_781_s_165	12845604	Finally, YPL261c and Sps2 (a protein with homology to GPI protein Ecm33), which  were also identified in their screen for GPI proteins, were excluded from our GPI  protein list because their N-terminal regions are unlikely to be signal peptides  for secretion.	gene_phenotype
68432	4	333304	7	NULL	NULL	NULL	NULL	Sps2	GP		does not have					signal peptides	GP		N-terminal residues		NULL		NULL	NULL	NULL	NULL	gw70_yeast_20_9_781_s_165	12845604	Finally, YPL261c and Sps2 (a protein with homology to GPI protein Ecm33), which  were also identified in their screen for GPI proteins, were excluded from our GPI  protein list because their N-terminal regions are unlikely to be signal peptides  for secretion.	gene_phenotype
68433	3	333304	7	NULL	NULL	NULL	NULL	signal peptides	GP		required for					secretion	Process				NULL		NULL	NULL	NULL	NULL	gw70_yeast_20_9_781_s_165	12845604	Finally, YPL261c and Sps2 (a protein with homology to GPI protein Ecm33), which  were also identified in their screen for GPI proteins, were excluded from our GPI  protein list because their N-terminal regions are unlikely to be signal peptides  for secretion.	gene_phenotype
68434	1	333306	7	NULL	NULL	0	NULL	mde7 	GP		induced during					meiosis	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_157_4_1469_s_146	11290704	These include an  S. cerevisiae gene we have named  WHI4 (YDL224c, see below) and two genes from  S. pombe, named SPCC16C4.07 (about which nothing is known) and  mde7 (induced during meiosis in a  mei4-dependent fashion,   A BE and SHIMODA 2000   ; PombePD, Proteome;	gene_phenotype
68435	2	333306	7	NULL	NULL	0	NULL	statement 1	Process		depends on					mei4	GP				NULL		0	NULL	NULL	NULL	gw60_genetics_157_4_1469_s_146	11290704	These include an  S. cerevisiae gene we have named  WHI4 (YDL224c, see below) and two genes from  S. pombe, named SPCC16C4.07 (about which nothing is known) and  mde7 (induced during meiosis in a  mei4-dependent fashion,   A BE and SHIMODA 2000   ; PombePD, Proteome;	gene_phenotype
68436	1	333307	7	NULL	NULL	0	NULL	YDR260c	GP		encode					protein	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_3_2118_s_99	10022899	These results thus suggested that the lack of the protein encoded by  YDR260c was responsible for the sporulation defect initially attributed by us to the  exg2 mutation.	gene_phenotype
68437	2	333307	7	NULL	NULL	NULL	NULL	statement 1	GP	lack of	is responsible for					sporulation defect	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_2118_s_99	10022899	These results thus suggested that the lack of the protein encoded by  YDR260c was responsible for the sporulation defect initially attributed by us to the  exg2 mutation.	gene_phenotype
68438	1	333308	7	NULL	NULL	0	NULL	plasmid pJC5	NucleicAcid		carry					EXG2 gene	GP	full-length			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_3_2118_s_98	10022899	Our results indicated that plasmid pJC5, carrying the full-length  EXG2 gene, was unable to complement the sporulation defect, while plasmids pRN30 (carrying  YDR260c and part of the 3' end of the  EXG2 coding sequence) and pPS47 (carrying only  YDR260c) restored the ability to form spores in the homozygous diploid mutant strain (Fig.  1).	gene_phenotype
68439	2	333308	7	NULL	NULL	0	NULL	statement 1	Process		unable to complement					sporulation defect	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_3_2118_s_98	10022899	Our results indicated that plasmid pJC5, carrying the full-length  EXG2 gene, was unable to complement the sporulation defect, while plasmids pRN30 (carrying  YDR260c and part of the 3' end of the  EXG2 coding sequence) and pPS47 (carrying only  YDR260c) restored the ability to form spores in the homozygous diploid mutant strain (Fig.  1).	gene_phenotype
68440	3	333308	7	NULL	NULL	0	NULL	plasmids pRN30	NucleicAcid		carry					YDR260c	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_3_2118_s_98	10022899	Our results indicated that plasmid pJC5, carrying the full-length  EXG2 gene, was unable to complement the sporulation defect, while plasmids pRN30 (carrying  YDR260c and part of the 3' end of the  EXG2 coding sequence) and pPS47 (carrying only  YDR260c) restored the ability to form spores in the homozygous diploid mutant strain (Fig.  1).	gene_phenotype
68441	4	333308	7	NULL	NULL	0	NULL	plasmids pRN30	NucleicAcid		carry					EXG2	GP		 part of the 3' end of coding sequence		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_3_2118_s_98	10022899	Our results indicated that plasmid pJC5, carrying the full-length  EXG2 gene, was unable to complement the sporulation defect, while plasmids pRN30 (carrying  YDR260c and part of the 3' end of the  EXG2 coding sequence) and pPS47 (carrying only  YDR260c) restored the ability to form spores in the homozygous diploid mutant strain (Fig.  1).	gene_phenotype
68442	5	333308	7	NULL	NULL	0	NULL	statement 3	Process		occur along with					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_3_2118_s_98	10022899	Our results indicated that plasmid pJC5, carrying the full-length  EXG2 gene, was unable to complement the sporulation defect, while plasmids pRN30 (carrying  YDR260c and part of the 3' end of the  EXG2 coding sequence) and pPS47 (carrying only  YDR260c) restored the ability to form spores in the homozygous diploid mutant strain (Fig.  1).	gene_phenotype
68443	6	333308	7	NULL	NULL	0	NULL	statement 5	Process		restore					spores	OrganismPart	ability to form			NULL	homozygous diploid mutant strain	0	NULL	NULL	NULL	gw60_molcellbiol_19_3_2118_s_98	10022899	Our results indicated that plasmid pJC5, carrying the full-length  EXG2 gene, was unable to complement the sporulation defect, while plasmids pRN30 (carrying  YDR260c and part of the 3' end of the  EXG2 coding sequence) and pPS47 (carrying only  YDR260c) restored the ability to form spores in the homozygous diploid mutant strain (Fig.  1).	gene_phenotype
68444	7	333308	7	NULL	NULL	0	NULL	pPS47	NucleicAcid		carry					YDR260c	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_3_2118_s_98	10022899	Our results indicated that plasmid pJC5, carrying the full-length  EXG2 gene, was unable to complement the sporulation defect, while plasmids pRN30 (carrying  YDR260c and part of the 3' end of the  EXG2 coding sequence) and pPS47 (carrying only  YDR260c) restored the ability to form spores in the homozygous diploid mutant strain (Fig.  1).	gene_phenotype
68445	8	333308	7	NULL	NULL	NULL	NULL	statement 7	GP		restore					spores	OrganismPart	ability to form			NULL	homozygous diploid mutant strain	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_3_2118_s_98	10022899	Our results indicated that plasmid pJC5, carrying the full-length  EXG2 gene, was unable to complement the sporulation defect, while plasmids pRN30 (carrying  YDR260c and part of the 3' end of the  EXG2 coding sequence) and pPS47 (carrying only  YDR260c) restored the ability to form spores in the homozygous diploid mutant strain (Fig.  1).	gene_phenotype
68446	1	333310	7	NULL	NULL	0	NULL	 YER048w-a	GP	open reading frame	is					ISD11	GP				NULL		0	NULL	NULL	NULL	gw70_embo_25_1_184_s_32	16341089	The open reading frame YER048w-a, now termed  ISD11, was found to be essential for cell viability in a sporulation approach and code  for an 11 kDa protein with mitochondrial localization (  et al;   et al).	gene_phenotype
68447	2	333310	7	NULL	NULL	0	NULL	statement 1	Process		is essential for					cell viability	Process				NULL		0	NULL	NULL	NULL	gw70_embo_25_1_184_s_32	16341089	The open reading frame YER048w-a, now termed  ISD11, was found to be essential for cell viability in a sporulation approach and code  for an 11 kDa protein with mitochondrial localization (  et al;   et al).	gene_phenotype
68448	3	333310	7	NULL	NULL	0	NULL	statement 2	Process		occur in a					sporulation approach	Process				NULL		0	NULL	NULL	NULL	gw70_embo_25_1_184_s_32	16341089	The open reading frame YER048w-a, now termed  ISD11, was found to be essential for cell viability in a sporulation approach and code  for an 11 kDa protein with mitochondrial localization (  et al;   et al).	gene_phenotype
68449	1	333311	7	NULL	NULL	0	NULL	ORF YER048w-a	GP	S. cerevisiae	essential for					viability	Process				NULL		0	NULL	NULL	NULL	gw70_embo_25_1_174_s_32	16341090	The ORF YER048w-a of  S. cerevisiae was reported to be essential for viability and encodes a mitochondrial protein with  a molecular mass of 11 kDa, further onwards referred to as Isd11 (ISC biogenesis  desulfurase interacting protein).	gene_phenotype
68450	2	333311	7	NULL	NULL	0	NULL	ORF YER048w-a	GP	S. cerevisiae	encode					Isd11 	GP				NULL		0	NULL	NULL	NULL	gw70_embo_25_1_174_s_32	16341090	The ORF YER048w-a of  S. cerevisiae was reported to be essential for viability and encodes a mitochondrial protein with  a molecular mass of 11 kDa, further onwards referred to as Isd11 (ISC biogenesis  desulfurase interacting protein).	gene_phenotype
68451	3	333311	7	NULL	NULL	0	NULL	Isd11 	GP		is a type of					mitochondrial protein	GP				NULL		0	NULL	NULL	NULL	gw70_embo_25_1_174_s_32	16341090	The ORF YER048w-a of  S. cerevisiae was reported to be essential for viability and encodes a mitochondrial protein with  a molecular mass of 11 kDa, further onwards referred to as Isd11 (ISC biogenesis  desulfurase interacting protein).	gene_phenotype
68452	4	333311	7	NULL	NULL	0	NULL	Isd11 	GP		is 					ISC biogenesis desulfurase interacting protein	GP				NULL		0	NULL	NULL	NULL	gw70_embo_25_1_174_s_32	16341090	The ORF YER048w-a of  S. cerevisiae was reported to be essential for viability and encodes a mitochondrial protein with  a molecular mass of 11 kDa, further onwards referred to as Isd11 (ISC biogenesis  desulfurase interacting protein).	gene_phenotype
68453	1	333312	7	NULL	NULL	0	NULL	 isd11-deletion strain	GP		derived from					YPH499	Organism				NULL		0	NULL	NULL	NULL	gw70_embo_25_1_184_s_275	16341089	An  isd11-deletion strain (derived from YPH499) carrying a  URA3-plasmid with the  ISD11 (Yer048w-a FOMP6/EDI1) open reading frame was viable like yeast wild-type cells but was unable to grow  on 5-fluoroorotic acid, that is, the plasmid loss approach did not lead to a viable   isd11-deletion strain.	gene_phenotype
68454	2	333312	7	NULL	NULL	0	NULL	isd11-deletion strain	GP		carry					URA3-plasmid	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_embo_25_1_184_s_275	16341089	An  isd11-deletion strain (derived from YPH499) carrying a  URA3-plasmid with the  ISD11 (Yer048w-a FOMP6/EDI1) open reading frame was viable like yeast wild-type cells but was unable to grow  on 5-fluoroorotic acid, that is, the plasmid loss approach did not lead to a viable   isd11-deletion strain.	gene_phenotype
68455	3	333312	7	NULL	NULL	0	NULL	URA3-plasmid	NucleicAcid		carry					ISD11	GP	open reading frame			NULL		0	NULL	NULL	NULL	gw70_embo_25_1_184_s_275	16341089	An  isd11-deletion strain (derived from YPH499) carrying a  URA3-plasmid with the  ISD11 (Yer048w-a FOMP6/EDI1) open reading frame was viable like yeast wild-type cells but was unable to grow  on 5-fluoroorotic acid, that is, the plasmid loss approach did not lead to a viable   isd11-deletion strain.	gene_phenotype
68456	4	333312	7	NULL	NULL	NULL	NULL	statement 3	Process	viability of	is similar to					wild-type cells	Cell	yeast			NULL		NULL	NULL	NULL	NULL	gw70_embo_25_1_184_s_275	16341089	An  isd11-deletion strain (derived from YPH499) carrying a  URA3-plasmid with the  ISD11 (Yer048w-a FOMP6/EDI1) open reading frame was viable like yeast wild-type cells but was unable to grow  on 5-fluoroorotic acid, that is, the plasmid loss approach did not lead to a viable   isd11-deletion strain.	gene_phenotype
68458	5	333312	7	NULL	NULL	NULL	NULL	statement 4	Process		unable to grow on					5-fluoroorotic acid	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_embo_25_1_184_s_275	16341089	An  isd11-deletion strain (derived from YPH499) carrying a  URA3-plasmid with the  ISD11 (Yer048w-a FOMP6/EDI1) open reading frame was viable like yeast wild-type cells but was unable to grow  on 5-fluoroorotic acid, that is, the plasmid loss approach did not lead to a viable   isd11-deletion strain.	gene_phenotype
68459	1	333314	7	NULL	NULL	0	NULL	BUD27	GP		possess					random budding patterns	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_163_3_875_s_167	12663529	Two of these genes,  BUD27 (YFL023W) and  BUD30 (YDL151C), have random budding patterns when mutated ( N I and SNYDER 2001   ), and both are hypersensitive to killer toxin.	gene_phenotype
68460	2	333314	7	NULL	NULL	0	NULL	BUD30	GP		possess					random budding patterns	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_163_3_875_s_167	12663529	Two of these genes,  BUD27 (YFL023W) and  BUD30 (YDL151C), have random budding patterns when mutated ( N I and SNYDER 2001   ), and both are hypersensitive to killer toxin.	gene_phenotype
68461	3	333314	7	NULL	NULL	0	NULL	statement 1	Process		occur upon					mutation	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_163_3_875_s_167	12663529	Two of these genes,  BUD27 (YFL023W) and  BUD30 (YDL151C), have random budding patterns when mutated ( N I and SNYDER 2001   ), and both are hypersensitive to killer toxin.	gene_phenotype
68462	4	333314	7	NULL	NULL	0	NULL	statement 2	Process		occur upon					mutation	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_163_3_875_s_167	12663529	Two of these genes,  BUD27 (YFL023W) and  BUD30 (YDL151C), have random budding patterns when mutated ( N I and SNYDER 2001   ), and both are hypersensitive to killer toxin.	gene_phenotype
68463	5	333314	7	NULL	NULL	0	NULL	BUD27	GP		is hypersensitive to					killer toxin	GP				NULL		0	NULL	NULL	NULL	gw60_genetics_163_3_875_s_167	12663529	Two of these genes,  BUD27 (YFL023W) and  BUD30 (YDL151C), have random budding patterns when mutated ( N I and SNYDER 2001   ), and both are hypersensitive to killer toxin.	gene_phenotype
68464	6	333314	7	NULL	NULL	0	NULL	BUD30	GP		is hypersensitive to					killer toxin	GP				NULL		0	NULL	NULL	NULL	gw60_genetics_163_3_875_s_167	12663529	Two of these genes,  BUD27 (YFL023W) and  BUD30 (YDL151C), have random budding patterns when mutated ( N I and SNYDER 2001   ), and both are hypersensitive to killer toxin.	gene_phenotype
68465	2	333315	7	NULL	NULL	NULL	NULL	Brp1	GP		bind					statement 1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_24267_s_99	15855155	On the other hand, neither Brp1 ( i.e. YGL007W, an open reading frame of unknown function) or Fes1p, a protein that binds to a complex involved in the regulation of protein translation, has any documented role in transport function ( ,  ,  ,  ).	gene_phenotype
68466	1	333315	7	NULL	NULL	NULL	NULL	complex	GP		involved in					protein translation	Process	regulation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_24267_s_99	15855155	On the other hand, neither Brp1 ( i.e. YGL007W, an open reading frame of unknown function) or Fes1p, a protein that binds to a complex involved in the regulation of protein translation, has any documented role in transport function ( ,  ,  ,  ).	gene_phenotype
68467	3	333315	7	NULL	NULL	0	NULL	Fes1p	GP		bind					statement 1	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_25_24267_s_99	15855155	On the other hand, neither Brp1 ( i.e. YGL007W, an open reading frame of unknown function) or Fes1p, a protein that binds to a complex involved in the regulation of protein translation, has any documented role in transport function ( ,  ,  ,  ).	gene_phenotype
68468	1	333316	7	NULL	NULL	0	NULL	FYV4 YHR059w	GP		is required for					viability	Process	yeast			NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_306	15334557	FYV4   YHR059w Required for yeast viability on toxin exposure	gene_phenotype
68469	2	333316	7	NULL	NULL	0	NULL	statement 1	Process		occur upon					toxin	GP	exposure to			NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_306	15334557	FYV4   YHR059w Required for yeast viability on toxin exposure	gene_phenotype
68470	1	333317	7	NULL	NULL	0	NULL	YKL195w/ FMP15	GP		encode					MIA40	GP				NULL		0	NULL	NULL	NULL	gw70_embo_23_19_3735_s_277	15359280	Conditional mutants of  MIA40 (encoded by YKL195w/ FMP15) were generated by error-prone PCR and isolated by screening for a temperature-sensitive  growth phenotype according to the procedure described in   et al.	gene_phenotype
68471	1	333318	7	NULL	NULL	NULL	NULL	YGL068W	GP	deletion of	results in					cell cycle	Process	arrest of specific phase of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_7_3946_s_158	11274415	Of the 36 hypothetical ORFs identified in our screen, deletion of three of them ( YGL068W,  YPL063W,  YKL195W) resulted in arrest in a specific phase of the cell cycle, reflecting a role for these gene products in cell cycle progression.	gene_phenotype
68472	2	333318	7	NULL	NULL	NULL	NULL	 YPL063W	GP	deletion of	results in					cell cycle	Process	arrest of specific phase of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_7_3946_s_158	11274415	Of the 36 hypothetical ORFs identified in our screen, deletion of three of them ( YGL068W,  YPL063W,  YKL195W) resulted in arrest in a specific phase of the cell cycle, reflecting a role for these gene products in cell cycle progression.	gene_phenotype
68473	3	333318	7	NULL	NULL	0	NULL	YKL195W	GP	deletion of	results in					cell cycle	Process	arrest of specific phase of			NULL		0	NULL	NULL	NULL	gw60_pnas_98_7_3946_s_158	11274415	Of the 36 hypothetical ORFs identified in our screen, deletion of three of them ( YGL068W,  YPL063W,  YKL195W) resulted in arrest in a specific phase of the cell cycle, reflecting a role for these gene products in cell cycle progression.	gene_phenotype
68474	4	333318	7	NULL	NULL	NULL	NULL	YGL068W	GP		play a role in					cell cycle	Process	progression of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_7_3946_s_158	11274415	Of the 36 hypothetical ORFs identified in our screen, deletion of three of them ( YGL068W,  YPL063W,  YKL195W) resulted in arrest in a specific phase of the cell cycle, reflecting a role for these gene products in cell cycle progression.	gene_phenotype
68475	5	333318	7	NULL	NULL	0	NULL	YPL063W	GP		play a role in					cell cycle	Process	progression of			NULL		0	NULL	NULL	NULL	gw60_pnas_98_7_3946_s_158	11274415	Of the 36 hypothetical ORFs identified in our screen, deletion of three of them ( YGL068W,  YPL063W,  YKL195W) resulted in arrest in a specific phase of the cell cycle, reflecting a role for these gene products in cell cycle progression.	gene_phenotype
68476	6	333318	7	NULL	NULL	0	NULL	YKL195W	GP		play a role in					cell cycle	Process	progression of			NULL		0	NULL	NULL	NULL	gw60_pnas_98_7_3946_s_158	11274415	Of the 36 hypothetical ORFs identified in our screen, deletion of three of them ( YGL068W,  YPL063W,  YKL195W) resulted in arrest in a specific phase of the cell cycle, reflecting a role for these gene products in cell cycle progression.	gene_phenotype
68477	7	333318	7	NULL	NULL	0	NULL	statement 1	Process		reflect					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_98_7_3946_s_158	11274415	Of the 36 hypothetical ORFs identified in our screen, deletion of three of them ( YGL068W,  YPL063W,  YKL195W) resulted in arrest in a specific phase of the cell cycle, reflecting a role for these gene products in cell cycle progression.	gene_phenotype
68478	8	333318	7	NULL	NULL	0	NULL	statement 2	Process		reflect					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_98_7_3946_s_158	11274415	Of the 36 hypothetical ORFs identified in our screen, deletion of three of them ( YGL068W,  YPL063W,  YKL195W) resulted in arrest in a specific phase of the cell cycle, reflecting a role for these gene products in cell cycle progression.	gene_phenotype
68479	9	333318	7	NULL	NULL	0	NULL	statement 3	Process		reflect					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_98_7_3946_s_158	11274415	Of the 36 hypothetical ORFs identified in our screen, deletion of three of them ( YGL068W,  YPL063W,  YKL195W) resulted in arrest in a specific phase of the cell cycle, reflecting a role for these gene products in cell cycle progression.	gene_phenotype
68480	1	333319	7	NULL	NULL	0	NULL	YGL068W	GP	deletion of	result in					inviable microcolonies	Organism				NULL		0	NULL	NULL	NULL	gw60_pnas_98_7_3946_s_112	11274415	Indicative of a cdc phenotype, deletion of each of the three ORFs,  YGL068W,  YKL195W, and  YPL063W resulted in inviable microcolonies that were comprised of 90, 84, and 100% unbudded cells, respectively, whereas the population of unbudded cells in matched wild-type colonies was 52% (Table  3).	gene_phenotype
68481	2	333319	7	NULL	NULL	0	NULL	YKL195W	GP	deletion of	result in					inviable microcolonies	Organism				NULL		0	NULL	NULL	NULL	gw60_pnas_98_7_3946_s_112	11274415	Indicative of a cdc phenotype, deletion of each of the three ORFs,  YGL068W,  YKL195W, and  YPL063W resulted in inviable microcolonies that were comprised of 90, 84, and 100% unbudded cells, respectively, whereas the population of unbudded cells in matched wild-type colonies was 52% (Table  3).	gene_phenotype
68482	3	333319	7	NULL	NULL	0	NULL	YPL063W	GP	deletion of	result in					inviable microcolonies	Organism				NULL		0	NULL	NULL	NULL	gw60_pnas_98_7_3946_s_112	11274415	Indicative of a cdc phenotype, deletion of each of the three ORFs,  YGL068W,  YKL195W, and  YPL063W resulted in inviable microcolonies that were comprised of 90, 84, and 100% unbudded cells, respectively, whereas the population of unbudded cells in matched wild-type colonies was 52% (Table  3).	gene_phenotype
68483	4	333319	7	NULL	NULL	0	NULL	statement 1	Process		is indicative of					cdc phenotype	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_98_7_3946_s_112	11274415	Indicative of a cdc phenotype, deletion of each of the three ORFs,  YGL068W,  YKL195W, and  YPL063W resulted in inviable microcolonies that were comprised of 90, 84, and 100% unbudded cells, respectively, whereas the population of unbudded cells in matched wild-type colonies was 52% (Table  3).	gene_phenotype
68484	5	333319	7	NULL	NULL	0	NULL	statement 2	Process		is indicative of					cdc phenotype	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_98_7_3946_s_112	11274415	Indicative of a cdc phenotype, deletion of each of the three ORFs,  YGL068W,  YKL195W, and  YPL063W resulted in inviable microcolonies that were comprised of 90, 84, and 100% unbudded cells, respectively, whereas the population of unbudded cells in matched wild-type colonies was 52% (Table  3).	gene_phenotype
68485	6	333319	7	NULL	NULL	0	NULL	statement 3	Process		is indicative of					cdc phenotype	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_98_7_3946_s_112	11274415	Indicative of a cdc phenotype, deletion of each of the three ORFs,  YGL068W,  YKL195W, and  YPL063W resulted in inviable microcolonies that were comprised of 90, 84, and 100% unbudded cells, respectively, whereas the population of unbudded cells in matched wild-type colonies was 52% (Table  3).	gene_phenotype
68486	7	333319	7	NULL	NULL	0	NULL	inviable microcolonies	Organism		comprise of					unbudded cells	Cell				NULL		0	NULL	NULL	NULL	gw60_pnas_98_7_3946_s_112	11274415	Indicative of a cdc phenotype, deletion of each of the three ORFs,  YGL068W,  YKL195W, and  YPL063W resulted in inviable microcolonies that were comprised of 90, 84, and 100% unbudded cells, respectively, whereas the population of unbudded cells in matched wild-type colonies was 52% (Table  3).	gene_phenotype
68487	1	333320	7	NULL	NULL	0	NULL	EAP1	GP		is expressed					constitutively	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_13_4604_s_300	10848587	EAP1 (ORF YKL204w) is constitutively expressed at low levels (100 to 1,000 times less than actin mRNA [ 68]) and is not differentially regulated during batch growth, throughout the cell cycle, or during sporulation, based on yeast gene expression databases ( 21,  26,  68,  73,  78; SGD [see above]; P. O. Brown laboratory, Stanford University [ http://cmgm.stanford.	gene_phenotype
68488	2	333320	7	NULL	NULL	NULL	NULL	EAP1	GP		 not regulated during		differentially			batch growth	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4604_s_300	10848587	EAP1 (ORF YKL204w) is constitutively expressed at low levels (100 to 1,000 times less than actin mRNA [ 68]) and is not differentially regulated during batch growth, throughout the cell cycle, or during sporulation, based on yeast gene expression databases ( 21,  26,  68,  73,  78; SGD [see above]; P. O. Brown laboratory, Stanford University [ http://cmgm.stanford.	gene_phenotype
68489	3	333320	7	NULL	NULL	0	NULL	statement 2	Process		occur throughout					cell cycle	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_13_4604_s_300	10848587	EAP1 (ORF YKL204w) is constitutively expressed at low levels (100 to 1,000 times less than actin mRNA [ 68]) and is not differentially regulated during batch growth, throughout the cell cycle, or during sporulation, based on yeast gene expression databases ( 21,  26,  68,  73,  78; SGD [see above]; P. O. Brown laboratory, Stanford University [ http://cmgm.stanford.	gene_phenotype
68490	4	333320	7	NULL	NULL	NULL	NULL	statement 2	Process		occur during					sporulation	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4604_s_300	10848587	EAP1 (ORF YKL204w) is constitutively expressed at low levels (100 to 1,000 times less than actin mRNA [ 68]) and is not differentially regulated during batch growth, throughout the cell cycle, or during sporulation, based on yeast gene expression databases ( 21,  26,  68,  73,  78; SGD [see above]; P. O. Brown laboratory, Stanford University [ http://cmgm.stanford.	gene_phenotype
68491	5	333320	7	NULL	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_13_4604_s_300	10848587	EAP1 (ORF YKL204w) is constitutively expressed at low levels (100 to 1,000 times less than actin mRNA [ 68]) and is not differentially regulated during batch growth, throughout the cell cycle, or during sporulation, based on yeast gene expression databases ( 21,  26,  68,  73,  78; SGD [see above]; P. O. Brown laboratory, Stanford University [ http://cmgm.stanford.	gene_phenotype
68492	6	333320	7	NULL	NULL	NULL	NULL	EAP1	GP	constitutive expression of	is less than					actin mRNA	NucleicAcid	constitutive expression of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_13_4604_s_300	10848587	EAP1 (ORF YKL204w) is constitutively expressed at low levels (100 to 1,000 times less than actin mRNA [ 68]) and is not differentially regulated during batch growth, throughout the cell cycle, or during sporulation, based on yeast gene expression databases ( 21,  26,  68,  73,  78; SGD [see above]; P. O. Brown laboratory, Stanford University [ http://cmgm.stanford.	gene_phenotype
68541	1	333321	7	NULL	NULL	NULL	NULL	Gic2	GP		is a component of					vesicular transport machinery	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biochem-j_365_pt-1_11931638_s_4	11931638	We also identified  components of the vesicular transport machinery such as Gic2 and Msb3,  proteins involved in transcriptional regulation such as Mbf1, Gcr2 and  Reg2, and a variety of other different proteins (Ppt1, Lre1, Rps0A and  Ylr177w).	gene_phenotype
68542	2	333321	7	NULL	NULL	0	NULL	 Msb3	GP		is a component of					vesicular transport machinery	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_biochem-j_365_pt-1_11931638_s_4	11931638	We also identified  components of the vesicular transport machinery such as Gic2 and Msb3,  proteins involved in transcriptional regulation such as Mbf1, Gcr2 and  Reg2, and a variety of other different proteins (Ppt1, Lre1, Rps0A and  Ylr177w).	gene_phenotype
68543	3	333321	7	NULL	NULL	0	NULL	Mbf1	GP		is involved in					transcriptional regulation	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_biochem-j_365_pt-1_11931638_s_4	11931638	We also identified  components of the vesicular transport machinery such as Gic2 and Msb3,  proteins involved in transcriptional regulation such as Mbf1, Gcr2 and  Reg2, and a variety of other different proteins (Ppt1, Lre1, Rps0A and  Ylr177w).	gene_phenotype
68544	4	333321	7	NULL	NULL	0	NULL	Gcr2	GP		is involved in					transcriptional regulation	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_biochem-j_365_pt-1_11931638_s_4	11931638	We also identified  components of the vesicular transport machinery such as Gic2 and Msb3,  proteins involved in transcriptional regulation such as Mbf1, Gcr2 and  Reg2, and a variety of other different proteins (Ppt1, Lre1, Rps0A and  Ylr177w).	gene_phenotype
68545	5	333321	7	NULL	NULL	0	NULL	Reg2	GP		is involved in					transcriptional regulation	GP				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_biochem-j_365_pt-1_11931638_s_4	11931638	We also identified  components of the vesicular transport machinery such as Gic2 and Msb3,  proteins involved in transcriptional regulation such as Mbf1, Gcr2 and  Reg2, and a variety of other different proteins (Ppt1, Lre1, Rps0A and  Ylr177w).	gene_phenotype
68546	1	333322	7	NULL	NULL	0	NULL	YOR049C	GP		is a type of					transporter gene family	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4020_s_122	11054416	It is quite possible, however, that increased expression of an as yet uncharacterized member of the transporter gene family, such as  YOR049C, could mediate the resistance of petite strains to 4-NQO.	gene_phenotype
68547	2	333322	7	NULL	NULL	0	NULL	petite strains	Organism		resistant to					4-NQO	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4020_s_122	11054416	It is quite possible, however, that increased expression of an as yet uncharacterized member of the transporter gene family, such as  YOR049C, could mediate the resistance of petite strains to 4-NQO.	gene_phenotype
68548	3	333322	7	NULL	NULL	0	NULL	YOR049C	GP		mediate		could			statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4020_s_122	11054416	It is quite possible, however, that increased expression of an as yet uncharacterized member of the transporter gene family, such as  YOR049C, could mediate the resistance of petite strains to 4-NQO.	gene_phenotype
68549	1	333323	7	NULL	NULL	0	NULL	 yeast cells 	Cell		lacks 					mitochondrial DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4020_s_181	11054416	Our studies support such a hypothesis; yeast cells lacking mitochondrial DNA acquire a multidrug-resistant phenotype perhaps as a result of increased expression of genes coding for membrane transporters ( e.g. PDR5 and  YOR049C) and show increased expression of genes coding for a number of cell surface proteins ( e.g. Hsp150, Sed1, and Cwp1) that may account for the changes in cell surface characteristics reported by Wilkie  et al. ( 70).	gene_phenotype
68550	2	333323	7	NULL	NULL	0	NULL	statement 1	Process		acquire					multidrug-resistance phenotype	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4020_s_181	11054416	Our studies support such a hypothesis; yeast cells lacking mitochondrial DNA acquire a multidrug-resistant phenotype perhaps as a result of increased expression of genes coding for membrane transporters ( e.g. PDR5 and  YOR049C) and show increased expression of genes coding for a number of cell surface proteins ( e.g. Hsp150, Sed1, and Cwp1) that may account for the changes in cell surface characteristics reported by Wilkie  et al. ( 70).	gene_phenotype
68551	3	333323	7	NULL	NULL	0	NULL	PDR5	GP		is a type of					membrane transporter	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4020_s_181	11054416	Our studies support such a hypothesis; yeast cells lacking mitochondrial DNA acquire a multidrug-resistant phenotype perhaps as a result of increased expression of genes coding for membrane transporters ( e.g. PDR5 and  YOR049C) and show increased expression of genes coding for a number of cell surface proteins ( e.g. Hsp150, Sed1, and Cwp1) that may account for the changes in cell surface characteristics reported by Wilkie  et al. ( 70).	gene_phenotype
68552	4	333323	7	NULL	NULL	0	NULL	YOR049C	GP		is a type of					membrane transporter	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4020_s_181	11054416	Our studies support such a hypothesis; yeast cells lacking mitochondrial DNA acquire a multidrug-resistant phenotype perhaps as a result of increased expression of genes coding for membrane transporters ( e.g. PDR5 and  YOR049C) and show increased expression of genes coding for a number of cell surface proteins ( e.g. Hsp150, Sed1, and Cwp1) that may account for the changes in cell surface characteristics reported by Wilkie  et al. ( 70).	gene_phenotype
68553	5	333323	7	NULL	NULL	0	NULL	statement 2	Process		because of					statement 3	Process	increased expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4020_s_181	11054416	Our studies support such a hypothesis; yeast cells lacking mitochondrial DNA acquire a multidrug-resistant phenotype perhaps as a result of increased expression of genes coding for membrane transporters ( e.g. PDR5 and  YOR049C) and show increased expression of genes coding for a number of cell surface proteins ( e.g. Hsp150, Sed1, and Cwp1) that may account for the changes in cell surface characteristics reported by Wilkie  et al. ( 70).	gene_phenotype
68554	6	333323	7	NULL	NULL	0	NULL	statement 2	Process		because of					statement 4	Process	increased expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4020_s_181	11054416	Our studies support such a hypothesis; yeast cells lacking mitochondrial DNA acquire a multidrug-resistant phenotype perhaps as a result of increased expression of genes coding for membrane transporters ( e.g. PDR5 and  YOR049C) and show increased expression of genes coding for a number of cell surface proteins ( e.g. Hsp150, Sed1, and Cwp1) that may account for the changes in cell surface characteristics reported by Wilkie  et al. ( 70).	gene_phenotype
68555	7	333323	7	NULL	NULL	0	NULL	Hsp150	GP		is a type of					cell surface proteins	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4020_s_181	11054416	Our studies support such a hypothesis; yeast cells lacking mitochondrial DNA acquire a multidrug-resistant phenotype perhaps as a result of increased expression of genes coding for membrane transporters ( e.g. PDR5 and  YOR049C) and show increased expression of genes coding for a number of cell surface proteins ( e.g. Hsp150, Sed1, and Cwp1) that may account for the changes in cell surface characteristics reported by Wilkie  et al. ( 70).	gene_phenotype
68556	8	333323	7	NULL	NULL	0	NULL	Sed1	GP		is a type of					cell surface protein	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4020_s_181	11054416	Our studies support such a hypothesis; yeast cells lacking mitochondrial DNA acquire a multidrug-resistant phenotype perhaps as a result of increased expression of genes coding for membrane transporters ( e.g. PDR5 and  YOR049C) and show increased expression of genes coding for a number of cell surface proteins ( e.g. Hsp150, Sed1, and Cwp1) that may account for the changes in cell surface characteristics reported by Wilkie  et al. ( 70).	gene_phenotype
68557	9	333323	7	NULL	NULL	0	NULL	Cwp1	GP		is a type of					cell surface protein	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4020_s_181	11054416	Our studies support such a hypothesis; yeast cells lacking mitochondrial DNA acquire a multidrug-resistant phenotype perhaps as a result of increased expression of genes coding for membrane transporters ( e.g. PDR5 and  YOR049C) and show increased expression of genes coding for a number of cell surface proteins ( e.g. Hsp150, Sed1, and Cwp1) that may account for the changes in cell surface characteristics reported by Wilkie  et al. ( 70).	gene_phenotype
68558	10	333323	7	NULL	NULL	0	NULL	Hsp150	GP		account for					cell surface	CellComponent	changes in characterisitics of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4020_s_181	11054416	Our studies support such a hypothesis; yeast cells lacking mitochondrial DNA acquire a multidrug-resistant phenotype perhaps as a result of increased expression of genes coding for membrane transporters ( e.g. PDR5 and  YOR049C) and show increased expression of genes coding for a number of cell surface proteins ( e.g. Hsp150, Sed1, and Cwp1) that may account for the changes in cell surface characteristics reported by Wilkie  et al. ( 70).	gene_phenotype
68559	11	333323	7	NULL	NULL	0	NULL	Sed1	GP		account for					cell surface	CellComponent	changes in characterisitics of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4020_s_181	11054416	Our studies support such a hypothesis; yeast cells lacking mitochondrial DNA acquire a multidrug-resistant phenotype perhaps as a result of increased expression of genes coding for membrane transporters ( e.g. PDR5 and  YOR049C) and show increased expression of genes coding for a number of cell surface proteins ( e.g. Hsp150, Sed1, and Cwp1) that may account for the changes in cell surface characteristics reported by Wilkie  et al. ( 70).	gene_phenotype
68560	12	333323	7	NULL	NULL	0	NULL	 Cwp1	GP		account for					cell surface	CellComponent	changes in characterisitics of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4020_s_181	11054416	Our studies support such a hypothesis; yeast cells lacking mitochondrial DNA acquire a multidrug-resistant phenotype perhaps as a result of increased expression of genes coding for membrane transporters ( e.g. PDR5 and  YOR049C) and show increased expression of genes coding for a number of cell surface proteins ( e.g. Hsp150, Sed1, and Cwp1) that may account for the changes in cell surface characteristics reported by Wilkie  et al. ( 70).	gene_phenotype
68561	13	333323	7	NULL	NULL	0	NULL	statement 2	Process		because of					Hsp150	GP	increased expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4020_s_181	11054416	Our studies support such a hypothesis; yeast cells lacking mitochondrial DNA acquire a multidrug-resistant phenotype perhaps as a result of increased expression of genes coding for membrane transporters ( e.g. PDR5 and  YOR049C) and show increased expression of genes coding for a number of cell surface proteins ( e.g. Hsp150, Sed1, and Cwp1) that may account for the changes in cell surface characteristics reported by Wilkie  et al. ( 70).	gene_phenotype
68562	14	333323	7	NULL	NULL	0	NULL	statement 2	Process		because of					Sed1	GP	increased expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4020_s_181	11054416	Our studies support such a hypothesis; yeast cells lacking mitochondrial DNA acquire a multidrug-resistant phenotype perhaps as a result of increased expression of genes coding for membrane transporters ( e.g. PDR5 and  YOR049C) and show increased expression of genes coding for a number of cell surface proteins ( e.g. Hsp150, Sed1, and Cwp1) that may account for the changes in cell surface characteristics reported by Wilkie  et al. ( 70).	gene_phenotype
68563	15	333323	7	NULL	NULL	0	NULL	statement 2	Process		because of					Cwp1	GP	increased expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4020_s_181	11054416	Our studies support such a hypothesis; yeast cells lacking mitochondrial DNA acquire a multidrug-resistant phenotype perhaps as a result of increased expression of genes coding for membrane transporters ( e.g. PDR5 and  YOR049C) and show increased expression of genes coding for a number of cell surface proteins ( e.g. Hsp150, Sed1, and Cwp1) that may account for the changes in cell surface characteristics reported by Wilkie  et al. ( 70).	gene_phenotype
68564	1	333324	7	NULL	NULL	0	NULL	haploid filamentous growth	Process		induce					ORF YOR225W	GP	expression of			NULL		0	NULL	NULL	NULL	gw60_pnas_97_22_12369_s_139	11035792	Also overexpressed 5.6-fold is the ORF  YOR225W, which has been shown to be induced in haploid filamentous growth, where its mRNA level is significantly increased in cells overproducing Tec1p compared with  tec1 null mutants ( 22).	gene_phenotype
68566	3	333324	7	NULL	NULL	0	NULL	YOR225W mRNA	NucleicAcid		increased in		significantly			statement 2	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_97_22_12369_s_139	11035792	Also overexpressed 5.6-fold is the ORF  YOR225W, which has been shown to be induced in haploid filamentous growth, where its mRNA level is significantly increased in cells overproducing Tec1p compared with  tec1 null mutants ( 22).	gene_phenotype
68567	2	333324	7	NULL	NULL	0	NULL	cells	Cell		overproduce					Tec1p	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_97_22_12369_s_139	11035792	Also overexpressed 5.6-fold is the ORF  YOR225W, which has been shown to be induced in haploid filamentous growth, where its mRNA level is significantly increased in cells overproducing Tec1p compared with  tec1 null mutants ( 22).	gene_phenotype
68568	4	333324	7	NULL	NULL	NULL	NULL	cells	Cell		produce					tec1 null mutant	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_22_12369_s_139	11035792	Also overexpressed 5.6-fold is the ORF  YOR225W, which has been shown to be induced in haploid filamentous growth, where its mRNA level is significantly increased in cells overproducing Tec1p compared with  tec1 null mutants ( 22).	gene_phenotype
68653	1	333325	7	NULL	NULL	0	NULL	peroxisomes	CellComponent	functional	required for					oleate	Chemical	metabolism of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_158_2_259_s_113	12135984	Viable yeast stains containing individual deletions of  YPL112c or  YOR084w constructed by an international consortium of laboratories ( Winzeler et al., 1999) (obtained from Resgen) were assayed for growth in the presence of oleate (requiring functional peroxisomes and mitochondria for metabolism) or acetate (requiring only mitochondria) as the sole carbon source.	gene_phenotype
68654	2	333325	7	NULL	NULL	0	NULL	mitochondria	CellComponent		required for					oleate	Chemical	metabolism of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_158_2_259_s_113	12135984	Viable yeast stains containing individual deletions of  YPL112c or  YOR084w constructed by an international consortium of laboratories ( Winzeler et al., 1999) (obtained from Resgen) were assayed for growth in the presence of oleate (requiring functional peroxisomes and mitochondria for metabolism) or acetate (requiring only mitochondria) as the sole carbon source.	gene_phenotype
68655	3	333325	7	NULL	NULL	0	NULL	mitochondria	CellComponent		required for					acetate	Chemical	metabolism of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_158_2_259_s_113	12135984	Viable yeast stains containing individual deletions of  YPL112c or  YOR084w constructed by an international consortium of laboratories ( Winzeler et al., 1999) (obtained from Resgen) were assayed for growth in the presence of oleate (requiring functional peroxisomes and mitochondria for metabolism) or acetate (requiring only mitochondria) as the sole carbon source.	gene_phenotype
68656	1	333326	7	NULL	NULL	0	NULL	IkappaB	GP		is a type of					inhibitor protein	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_25_15494_s_25	9624136	The prototypical pathway involves its liberation from an inactive complex with the inhibitor protein, IkappaB, which resides in the cytosol ( 31,  32).	gene_phenotype
68657	2	333326	7	NULL	NULL	0	NULL	IkappaB	GP		resides in 					cytosol	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_25_15494_s_25	9624136	The prototypical pathway involves its liberation from an inactive complex with the inhibitor protein, IkappaB, which resides in the cytosol ( 31,  32).	gene_phenotype
68658	1	333328	7	NULL	NULL	0	NULL	Sir2	GP		repress					HMR-proximal loci	Chromosome				NULL		0	NULL	NULL	NULL	gw60_cell_112_5_725_s_111	12628191	It is notable that several of the  HMR-proximal loci display repression by Sir2 in an  HTZ1+ genetic background (e.g.,  YCR106W in   Figure 3B), suggesting that a locus can be partially protected from silencing by Htz1; that is, in some cases, Htz1 may reduce but not eliminate heterochromatin formation.	gene_phenotype
68662	2	333328	7	NULL	NULL	0	NULL	statement 1	Process		occur in a					HTZ1+ 	GP	genetic background of			NULL		0	NULL	NULL	NULL	gw60_cell_112_5_725_s_111	12628191	It is notable that several of the  HMR-proximal loci display repression by Sir2 in an  HTZ1+ genetic background (e.g.,  YCR106W in   Figure 3B), suggesting that a locus can be partially protected from silencing by Htz1; that is, in some cases, Htz1 may reduce but not eliminate heterochromatin formation.	gene_phenotype
68663	3	333328	7	NULL	NULL	NULL	NULL	locus	Chromosome		protected from		partially			Htz1	GP	silencing by			NULL		NULL	NULL	NULL	NULL	gw60_cell_112_5_725_s_111	12628191	It is notable that several of the  HMR-proximal loci display repression by Sir2 in an  HTZ1+ genetic background (e.g.,  YCR106W in   Figure 3B), suggesting that a locus can be partially protected from silencing by Htz1; that is, in some cases, Htz1 may reduce but not eliminate heterochromatin formation.	gene_phenotype
68668	4	333328	7	NULL	NULL	0	NULL	statement 1	Process		suggests					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_cell_112_5_725_s_111	12628191	It is notable that several of the  HMR-proximal loci display repression by Sir2 in an  HTZ1+ genetic background (e.g.,  YCR106W in   Figure 3B), suggesting that a locus can be partially protected from silencing by Htz1; that is, in some cases, Htz1 may reduce but not eliminate heterochromatin formation.	gene_phenotype
68671	5	333328	7	NULL	NULL	0	NULL	Htz1	GP		eliminate		may			heterochromatin	Chromosome	formation of			NULL		0	NULL	NULL	NULL	gw60_cell_112_5_725_s_111	12628191	It is notable that several of the  HMR-proximal loci display repression by Sir2 in an  HTZ1+ genetic background (e.g.,  YCR106W in   Figure 3B), suggesting that a locus can be partially protected from silencing by Htz1; that is, in some cases, Htz1 may reduce but not eliminate heterochromatin formation.	gene_phenotype
68673	6	333328	7	NULL	NULL	0	NULL	 Htz1	GP		does not eliminate					heterochromatin	Chromosome	formation of			NULL		0	NULL	NULL	NULL	gw60_cell_112_5_725_s_111	12628191	It is notable that several of the  HMR-proximal loci display repression by Sir2 in an  HTZ1+ genetic background (e.g.,  YCR106W in   Figure 3B), suggesting that a locus can be partially protected from silencing by Htz1; that is, in some cases, Htz1 may reduce but not eliminate heterochromatin formation.	gene_phenotype
68675	1	333330	7	NULL	NULL	0	NULL	HPR1 YDR183w	GP		suppress					intrachromosomal recombination	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_312	15334557	HPR1   YDR183w Suppresses intrachromosomal recombination; possibly also involved in RNA elongation  from polymerase II promoters and mRNA nuclear export	gene_phenotype
68676	2	333330	7	NULL	NULL	NULL	NULL	polymerase II	GP		elongates			promoter		RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_yeast_21_11_927_s_312	15334557	HPR1   YDR183w Suppresses intrachromosomal recombination; possibly also involved in RNA elongation  from polymerase II promoters and mRNA nuclear export	gene_phenotype
68677	3	333330	7	NULL	NULL	0	NULL	HPR1 YDR183w 	GP		involved in		possibly			statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_312	15334557	HPR1   YDR183w Suppresses intrachromosomal recombination; possibly also involved in RNA elongation  from polymerase II promoters and mRNA nuclear export	gene_phenotype
68678	4	333330	7	NULL	NULL	0	NULL	HPR1 YDR183w 	GP		is involved in					mRNA 	NucleicAcid	nuclear export of			NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_312	15334557	HPR1   YDR183w Suppresses intrachromosomal recombination; possibly also involved in RNA elongation  from polymerase II promoters and mRNA nuclear export	gene_phenotype
68683	1	333331	7	NULL	NULL	0	NULL	YDR236c 	GP		is essential for					growth	Process				NULL	YPD medium	0	NULL	NULL	NULL	gw60_jbiolchem_275_37_28618_s_102	10887197	When  ydr236cdelta/ YDR236c diploids were sporulated and the resulting tetrads dissected, viability segregated 2+:2  and all viable spores were geneticin-sensitive, suggesting that  YDR236c is a single copy gene that is essential for growth on YPD medium.	gene_phenotype
68684	1	333334	7	NULL	NULL	0	NULL	ADH 	GP		contains			promoter		ORF YEL003w 	GP				NULL		0	NULL	NULL	NULL	gw60_embo_17_4_952_s_62	9463374	Only the  ADH promoter fusion with the intron-containing ORF YEL003w complemented  gim4 cells (data not shown) .	gene_phenotype
68685	2	333334	7	NULL	NULL	0	NULL	statement 1	Process		complement					gim4 cells	Cell				NULL		0	NULL	NULL	NULL	gw60_embo_17_4_952_s_62	9463374	Only the  ADH promoter fusion with the intron-containing ORF YEL003w complemented  gim4 cells (data not shown) .	gene_phenotype
68686	1	333335	7	NULL	NULL	NULL	NULL	Ndt1p	GP		is a gene product of					YIL006W	GP				NULL	S.cerevisiae	NULL	NULL	NULL	NULL	gw70_jbiolchem_281_3_1524_s_26	16291748	In this study we provide evidence that the gene products of  YIL006W and  YEL006W, named Ndt1p and Ndt2p, respectively, are two isoforms of the mitochondrial NAD+ transporter in  S. cerevisiae.	gene_phenotype
68687	2	333335	7	NULL	NULL	NULL	NULL	Ndt2p	GP		is a gene product of					YEL006W	GP				NULL	S.cerevisiae	NULL	NULL	NULL	NULL	gw70_jbiolchem_281_3_1524_s_26	16291748	In this study we provide evidence that the gene products of  YIL006W and  YEL006W, named Ndt1p and Ndt2p, respectively, are two isoforms of the mitochondrial NAD+ transporter in  S. cerevisiae.	gene_phenotype
68688	3	333335	7	NULL	NULL	NULL	NULL	Ndt1p	GP		is an isoform of					Ndt2p	GP				NULL	S. cerevisiae	NULL	NULL	NULL	NULL	gw70_jbiolchem_281_3_1524_s_26	16291748	In this study we provide evidence that the gene products of  YIL006W and  YEL006W, named Ndt1p and Ndt2p, respectively, are two isoforms of the mitochondrial NAD+ transporter in  S. cerevisiae.	gene_phenotype
68690	4	333335	7	NULL	NULL	NULL	NULL	Ndt1p	GP		is a type of					mitochondrial NAD+ transporter	GP				NULL	S.cerevisiae	NULL	NULL	NULL	NULL	gw70_jbiolchem_281_3_1524_s_26	16291748	In this study we provide evidence that the gene products of  YIL006W and  YEL006W, named Ndt1p and Ndt2p, respectively, are two isoforms of the mitochondrial NAD+ transporter in  S. cerevisiae.	gene_phenotype
68691	5	333335	7	NULL	NULL	0	NULL	Ndt2p	GP		is a type of					mitochondrial NAD+ transporter	GP				NULL	S.cerevisiae	0	NULL	NULL	NULL	gw70_jbiolchem_281_3_1524_s_26	16291748	In this study we provide evidence that the gene products of  YIL006W and  YEL006W, named Ndt1p and Ndt2p, respectively, are two isoforms of the mitochondrial NAD+ transporter in  S. cerevisiae.	gene_phenotype
68694	1	333336	7	NULL	NULL	NULL	NULL	Rim2p	GP		transports					pyrimidine nucleotides	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1757_9_1249_s_284	16844075	The proteins encoded by YIL006w and YEL006w cluster in the phylogenetic tree of yeast  carriers with Rim2p and Flx1p, the transporters of pyrimidine nucleotides   [32] and FAD   [92], respectively, and so attempts to uncover their functions were predicated on the  assumption that they would transport nucleotide-type molecules also.	gene_phenotype
68696	2	333336	7	NULL	NULL	0	NULL	Flx1p	GP		transports					FAD	Chemical				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1757_9_1249_s_284	16844075	The proteins encoded by YIL006w and YEL006w cluster in the phylogenetic tree of yeast  carriers with Rim2p and Flx1p, the transporters of pyrimidine nucleotides   [32] and FAD   [92], respectively, and so attempts to uncover their functions were predicated on the  assumption that they would transport nucleotide-type molecules also.	gene_phenotype
68703	1	333338	7	NULL	NULL	0	NULL	YGL136c 	GP	deletion of	grew in		slowly			glycerol medium	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_yeast_16_7_10806424_s_7	10806424	Segregants bearing a deletion in YGL136c  grew slowly in complete glycerol medium at 37 degrees C. Cells deleted  in YGL133w showed abnormal morphology and reduced mating efficiency, but  these phenotypes were observed only when the YGL133w disruption was in  a MATalpha background.	gene_phenotype
68704	2	333338	7	NULL	NULL	NULL	NULL	YGL133w	GP	deletion of	shows					morphology		abnormal			NULL	cells	NULL	NULL	NULL	NULL	abs-batch0650-0679_yeast_16_7_10806424_s_7	10806424	Segregants bearing a deletion in YGL136c  grew slowly in complete glycerol medium at 37 degrees C. Cells deleted  in YGL133w showed abnormal morphology and reduced mating efficiency, but  these phenotypes were observed only when the YGL133w disruption was in  a MATalpha background.	gene_phenotype
68708	3	333338	7	NULL	NULL	0	NULL	YGL133w	GP	deletion of	reduced					mating 	Process	efficiency of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_yeast_16_7_10806424_s_7	10806424	Segregants bearing a deletion in YGL136c  grew slowly in complete glycerol medium at 37 degrees C. Cells deleted  in YGL133w showed abnormal morphology and reduced mating efficiency, but  these phenotypes were observed only when the YGL133w disruption was in  a MATalpha background.	gene_phenotype
68709	4	333338	7	NULL	NULL	0	NULL	statement 2	Process		occur in the					MATalpha	GP	background of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_yeast_16_7_10806424_s_7	10806424	Segregants bearing a deletion in YGL136c  grew slowly in complete glycerol medium at 37 degrees C. Cells deleted  in YGL133w showed abnormal morphology and reduced mating efficiency, but  these phenotypes were observed only when the YGL133w disruption was in  a MATalpha background.	gene_phenotype
68710	5	333338	7	NULL	NULL	0	NULL	statement 3	Process		occur in the 					MATalpha	GP	background of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_yeast_16_7_10806424_s_7	10806424	Segregants bearing a deletion in YGL136c  grew slowly in complete glycerol medium at 37 degrees C. Cells deleted  in YGL133w showed abnormal morphology and reduced mating efficiency, but  these phenotypes were observed only when the YGL133w disruption was in  a MATalpha background.	gene_phenotype
68711	1	333339	7	NULL	NULL	0	NULL	YGR203w	GP	deletion of	is					viable	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_101_36_13380_s_206	15329414	Deletion of YGR203w is viable but alters yeast fitness after 20 generations ( ).	gene_phenotype
68712	2	333339	7	NULL	NULL	0	NULL	YGR203w	GP	deletion of	alters					yeast	Organism	fitness of			NULL		0	NULL	NULL	NULL	gw70_pnas_101_36_13380_s_206	15329414	Deletion of YGR203w is viable but alters yeast fitness after 20 generations ( ).	gene_phenotype
68713	1	333340	7	NULL	NULL	NULL	NULL	CDC25 	GP		is homologous to					small CDC25-like protein	GP				NULL	yeast	NULL	NULL	NULL	NULL	gw70_pnas_101_36_13380_s_98	15329414	Arath;CDC25 is also homologous to small CDC25-like proteins found in yeast such as YGR203w from  S. cerevisiae or IBP1 from  Sch. pombe, where the latter was recently shown experimentally to display a tyrosine-phosphatase activity ( ).	gene_phenotype
68714	2	333340	7	NULL	NULL	NULL	NULL	YGR203w 	GP	S. cerevisiae	is a type of					small CDC25-like proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_36_13380_s_98	15329414	Arath;CDC25 is also homologous to small CDC25-like proteins found in yeast such as YGR203w from  S. cerevisiae or IBP1 from  Sch. pombe, where the latter was recently shown experimentally to display a tyrosine-phosphatase activity ( ).	gene_phenotype
68715	3	333340	7	NULL	NULL	0	NULL	IBP1	GP	Sch. pombe	is a type of					small CDC25-like protein	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_36_13380_s_98	15329414	Arath;CDC25 is also homologous to small CDC25-like proteins found in yeast such as YGR203w from  S. cerevisiae or IBP1 from  Sch. pombe, where the latter was recently shown experimentally to display a tyrosine-phosphatase activity ( ).	gene_phenotype
68716	4	333340	7	NULL	NULL	0	NULL	IBP1	GP		display					tyrosine-phosphatase activity	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_101_36_13380_s_98	15329414	Arath;CDC25 is also homologous to small CDC25-like proteins found in yeast such as YGR203w from  S. cerevisiae or IBP1 from  Sch. pombe, where the latter was recently shown experimentally to display a tyrosine-phosphatase activity ( ).	gene_phenotype
68723	1	333342	7	NULL	NULL	0	NULL	YIL083C gene	GP		essential for					viability	Process	yeast			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_24_21431_s_144	11923312	The YIL083C gene was found to be essential for yeast viability in a systematic gene knockout study (Saccharomyces Genome Database) (see Ref.  20), providing additional support for this functional prediction.	gene_phenotype
68724	1	333343	7	NULL	NULL	0	NULL	PRM1	GP		is linked to					membrane	CellComponent	biosynthesis of			NULL		0	NULL	NULL	NULL	gw70_genomeres_13_7_1706_s_133	12840046	The genes included  PRM1 (linked to  membrane biosynthesis),  FIG2, AGA1, FUS1 (cell fusion),  GIC2  (mating projection formation),  CIK1, KAR2 (nuclear fusion),  FUS3,  STE12, and  HYM1 (mating signaling) along with other genes of yet  unknown relevance ( YOR0343C, PEP1, SCH9, YIL036C, YIL083C, YOL155C).	gene_phenotype
68725	2	333343	7	NULL	NULL	0	NULL	FIG2	GP		is involved in					cell fusion	Process				NULL		0	NULL	NULL	NULL	gw70_genomeres_13_7_1706_s_133	12840046	The genes included  PRM1 (linked to  membrane biosynthesis),  FIG2, AGA1, FUS1 (cell fusion),  GIC2  (mating projection formation),  CIK1, KAR2 (nuclear fusion),  FUS3,  STE12, and  HYM1 (mating signaling) along with other genes of yet  unknown relevance ( YOR0343C, PEP1, SCH9, YIL036C, YIL083C, YOL155C).	gene_phenotype
68726	3	333343	7	NULL	NULL	0	NULL	AGA1	GP		is involved in					cell fusion	Process				NULL		0	NULL	NULL	NULL	gw70_genomeres_13_7_1706_s_133	12840046	The genes included  PRM1 (linked to  membrane biosynthesis),  FIG2, AGA1, FUS1 (cell fusion),  GIC2  (mating projection formation),  CIK1, KAR2 (nuclear fusion),  FUS3,  STE12, and  HYM1 (mating signaling) along with other genes of yet  unknown relevance ( YOR0343C, PEP1, SCH9, YIL036C, YIL083C, YOL155C).	gene_phenotype
68727	4	333343	7	NULL	NULL	0	NULL	FUS1	GP		is involved in					cell fusion	Process				NULL		0	NULL	NULL	NULL	gw70_genomeres_13_7_1706_s_133	12840046	The genes included  PRM1 (linked to  membrane biosynthesis),  FIG2, AGA1, FUS1 (cell fusion),  GIC2  (mating projection formation),  CIK1, KAR2 (nuclear fusion),  FUS3,  STE12, and  HYM1 (mating signaling) along with other genes of yet  unknown relevance ( YOR0343C, PEP1, SCH9, YIL036C, YIL083C, YOL155C).	gene_phenotype
68728	5	333343	7	NULL	NULL	0	NULL	GIC2	GP		is involved in					mating projection	Process	 formation of			NULL		0	NULL	NULL	NULL	gw70_genomeres_13_7_1706_s_133	12840046	The genes included  PRM1 (linked to  membrane biosynthesis),  FIG2, AGA1, FUS1 (cell fusion),  GIC2  (mating projection formation),  CIK1, KAR2 (nuclear fusion),  FUS3,  STE12, and  HYM1 (mating signaling) along with other genes of yet  unknown relevance ( YOR0343C, PEP1, SCH9, YIL036C, YIL083C, YOL155C).	gene_phenotype
68729	6	333343	7	NULL	NULL	0	NULL	CIK1	GP		is involved in					nuclear fusion	Process				NULL		0	NULL	NULL	NULL	gw70_genomeres_13_7_1706_s_133	12840046	The genes included  PRM1 (linked to  membrane biosynthesis),  FIG2, AGA1, FUS1 (cell fusion),  GIC2  (mating projection formation),  CIK1, KAR2 (nuclear fusion),  FUS3,  STE12, and  HYM1 (mating signaling) along with other genes of yet  unknown relevance ( YOR0343C, PEP1, SCH9, YIL036C, YIL083C, YOL155C).	gene_phenotype
68730	7	333343	7	NULL	NULL	0	NULL	KAR2	GP		is involved in					nuclear fusion	Process				NULL		0	NULL	NULL	NULL	gw70_genomeres_13_7_1706_s_133	12840046	The genes included  PRM1 (linked to  membrane biosynthesis),  FIG2, AGA1, FUS1 (cell fusion),  GIC2  (mating projection formation),  CIK1, KAR2 (nuclear fusion),  FUS3,  STE12, and  HYM1 (mating signaling) along with other genes of yet  unknown relevance ( YOR0343C, PEP1, SCH9, YIL036C, YIL083C, YOL155C).	gene_phenotype
68731	8	333343	7	NULL	NULL	0	NULL	FUS3	GP		is involved in					mating signaling	Process				NULL		0	NULL	NULL	NULL	gw70_genomeres_13_7_1706_s_133	12840046	The genes included  PRM1 (linked to  membrane biosynthesis),  FIG2, AGA1, FUS1 (cell fusion),  GIC2  (mating projection formation),  CIK1, KAR2 (nuclear fusion),  FUS3,  STE12, and  HYM1 (mating signaling) along with other genes of yet  unknown relevance ( YOR0343C, PEP1, SCH9, YIL036C, YIL083C, YOL155C).	gene_phenotype
68732	9	333343	7	NULL	NULL	0	NULL	STE12	GP		is involved in					mating signaling	Process				NULL		0	NULL	NULL	NULL	gw70_genomeres_13_7_1706_s_133	12840046	The genes included  PRM1 (linked to  membrane biosynthesis),  FIG2, AGA1, FUS1 (cell fusion),  GIC2  (mating projection formation),  CIK1, KAR2 (nuclear fusion),  FUS3,  STE12, and  HYM1 (mating signaling) along with other genes of yet  unknown relevance ( YOR0343C, PEP1, SCH9, YIL036C, YIL083C, YOL155C).	gene_phenotype
68733	10	333343	7	NULL	NULL	0	NULL	HYM1 	GP		is involved in					mating signaling	Process				NULL		0	NULL	NULL	NULL	gw70_genomeres_13_7_1706_s_133	12840046	The genes included  PRM1 (linked to  membrane biosynthesis),  FIG2, AGA1, FUS1 (cell fusion),  GIC2  (mating projection formation),  CIK1, KAR2 (nuclear fusion),  FUS3,  STE12, and  HYM1 (mating signaling) along with other genes of yet  unknown relevance ( YOR0343C, PEP1, SCH9, YIL036C, YIL083C, YOL155C).	gene_phenotype
68734	1	333344	7	NULL	NULL	0	NULL	14-3-3 protein	GP		mediate					anti-apoptotic signal	Process	essential			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_6_2201_s_269	12808022	14-3-3 proteins  mediate an essential anti-apoptotic signal.	gene_phenotype
68896	1	333345	7	NULL	NULL	0	NULL	HXT16	GP		is a type of					hexose transporter genes	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_1_437_s_235	15496405	The remaining 14 genes of the 35 genes of the discussed cluster were composed of two hexose transporter genes ( HXT16 and  HXT17), five genes encoding ribosomal proteins ( RSP10A, RPS25A, RPP1B, RPL4A, and  RPL9A), and seven genes belonging to different metabolic routes ( SUT1, OSH7, AGP1, IMD2, YLR089C, YAR075W, and  GPA1) ( Fig. 6,  middle panel).	gene_phenotype
68897	2	333345	7	NULL	NULL	0	NULL	HXT17	GP		is a type of					hexose transporter genes	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_1_437_s_235	15496405	The remaining 14 genes of the 35 genes of the discussed cluster were composed of two hexose transporter genes ( HXT16 and  HXT17), five genes encoding ribosomal proteins ( RSP10A, RPS25A, RPP1B, RPL4A, and  RPL9A), and seven genes belonging to different metabolic routes ( SUT1, OSH7, AGP1, IMD2, YLR089C, YAR075W, and  GPA1) ( Fig. 6,  middle panel).	gene_phenotype
68898	3	333345	7	NULL	NULL	NULL	NULL	RSP10A	GP		encode					ribosomal proteins 	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_1_437_s_235	15496405	The remaining 14 genes of the 35 genes of the discussed cluster were composed of two hexose transporter genes ( HXT16 and  HXT17), five genes encoding ribosomal proteins ( RSP10A, RPS25A, RPP1B, RPL4A, and  RPL9A), and seven genes belonging to different metabolic routes ( SUT1, OSH7, AGP1, IMD2, YLR089C, YAR075W, and  GPA1) ( Fig. 6,  middle panel).	gene_phenotype
68899	4	333345	7	NULL	NULL	0	NULL	RPS25A	GP		encode					ribosomal proteins	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_1_437_s_235	15496405	The remaining 14 genes of the 35 genes of the discussed cluster were composed of two hexose transporter genes ( HXT16 and  HXT17), five genes encoding ribosomal proteins ( RSP10A, RPS25A, RPP1B, RPL4A, and  RPL9A), and seven genes belonging to different metabolic routes ( SUT1, OSH7, AGP1, IMD2, YLR089C, YAR075W, and  GPA1) ( Fig. 6,  middle panel).	gene_phenotype
68900	5	333345	7	NULL	NULL	NULL	NULL	RPP1B	GP		encode					ribosomal proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_1_437_s_235	15496405	The remaining 14 genes of the 35 genes of the discussed cluster were composed of two hexose transporter genes ( HXT16 and  HXT17), five genes encoding ribosomal proteins ( RSP10A, RPS25A, RPP1B, RPL4A, and  RPL9A), and seven genes belonging to different metabolic routes ( SUT1, OSH7, AGP1, IMD2, YLR089C, YAR075W, and  GPA1) ( Fig. 6,  middle panel).	gene_phenotype
68901	6	333345	7	NULL	NULL	0	NULL	RPL4A	GP		encode					ribosomal proteins	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_1_437_s_235	15496405	The remaining 14 genes of the 35 genes of the discussed cluster were composed of two hexose transporter genes ( HXT16 and  HXT17), five genes encoding ribosomal proteins ( RSP10A, RPS25A, RPP1B, RPL4A, and  RPL9A), and seven genes belonging to different metabolic routes ( SUT1, OSH7, AGP1, IMD2, YLR089C, YAR075W, and  GPA1) ( Fig. 6,  middle panel).	gene_phenotype
68902	7	333345	7	NULL	NULL	0	NULL	RPL9A	GP		encode					ribosomal proteins	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_1_437_s_235	15496405	The remaining 14 genes of the 35 genes of the discussed cluster were composed of two hexose transporter genes ( HXT16 and  HXT17), five genes encoding ribosomal proteins ( RSP10A, RPS25A, RPP1B, RPL4A, and  RPL9A), and seven genes belonging to different metabolic routes ( SUT1, OSH7, AGP1, IMD2, YLR089C, YAR075W, and  GPA1) ( Fig. 6,  middle panel).	gene_phenotype
68903	1	333346	7	NULL	NULL	0	NULL	DH17	GP		is a type of					 C-terminal specific monoclonal antibody	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_30_27200_s_245	12004072	This was investigated by examining apoptotic HeLa-E cells with a C-terminal specific monoclonal antibody (DH17).	gene_phenotype
68904	1	333347	7	NULL	NULL	0	NULL	YNL026w	GP		is essential for					haploid progeny	Process	viability in			NULL		0	NULL	NULL	NULL	gw70_cellbiol_164_1_19_s_124	14699090	YNL026w is essential for viability in haploid progeny derived from IGY002.	gene_phenotype
68905	2	333347	7	NULL	NULL	0	NULL	YNL026w	GP		is derived from					IGY002	GP				NULL		0	NULL	NULL	NULL	gw70_cellbiol_164_1_19_s_124	14699090	YNL026w is essential for viability in haploid progeny derived from IGY002.	gene_phenotype
68906	1	333348	7	NULL	NULL	0	NULL	NAP-1	GP		is not essential for					S. cerevisiae	Organism	viability of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_40_25041_s_207	8798787	This NAP-1/SET-related ORF YNL246w protein may compensate for the absence of NAP-1 and thus be responsible, at least in part, for the observation that NAP-1 is not essential for viability of  S. cerevisiae ( 46).	gene_phenotype
68907	1	333349	7	NULL	NULL	0	NULL		Organism	yeast	harbor			patatin domain-containing proteins		lipolytic functions	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_491_s_271	16267052	Because three other patatin domain-containing proteins in yeast harbor lipolytic functions, including the phospholipase B activity of the neuropathy target esterase ortholog, Nte1 ( ,  ), a related enzymatic function for Yor081c appears likely.	gene_phenotype
68908	2	333349	7	NULL	NULL	0	NULL	Nte1	GP		activates					phospholipase B	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_491_s_271	16267052	Because three other patatin domain-containing proteins in yeast harbor lipolytic functions, including the phospholipase B activity of the neuropathy target esterase ortholog, Nte1 ( ,  ), a related enzymatic function for Yor081c appears likely.	gene_phenotype
68909	3	333349	7	NULL	NULL	NULL	NULL	 Nte1 	GP		is ortholog of					neuropathy target esterase	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_1_491_s_271	16267052	Because three other patatin domain-containing proteins in yeast harbor lipolytic functions, including the phospholipase B activity of the neuropathy target esterase ortholog, Nte1 ( ,  ), a related enzymatic function for Yor081c appears likely.	gene_phenotype
68910	1	333351	7	NULL	NULL	NULL	NULL	NKC6 cells	GP		produce					YOR071c	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_31_19165_s_123	9235906	As shown in Table  II, NKC6 cells producing YOR071c or YOR192c protein showed the thiamin transport activities of 13.7% and 41.0%, respectively, compared with the cells expressing THI10 protein.	gene_phenotype
68911	2	333351	7	NULL	NULL	0	NULL	NKC6 cells	GP		produce					YOR192c protein	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_31_19165_s_123	9235906	As shown in Table  II, NKC6 cells producing YOR071c or YOR192c protein showed the thiamin transport activities of 13.7% and 41.0%, respectively, compared with the cells expressing THI10 protein.	gene_phenotype
68912	3	333351	7	NULL	NULL	NULL	NULL	statement 1	Process		shows					 thiamin	Chemical	transport activities of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_31_19165_s_123	9235906	As shown in Table  II, NKC6 cells producing YOR071c or YOR192c protein showed the thiamin transport activities of 13.7% and 41.0%, respectively, compared with the cells expressing THI10 protein.	gene_phenotype
68913	4	333351	7	NULL	NULL	0	NULL	statement 2	Process		shows					thiamin	Chemical	transport activities of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_31_19165_s_123	9235906	As shown in Table  II, NKC6 cells producing YOR071c or YOR192c protein showed the thiamin transport activities of 13.7% and 41.0%, respectively, compared with the cells expressing THI10 protein.	gene_phenotype
68914	5	333351	7	NULL	NULL	0	NULL	Cells	Cell		express					THI10 protein	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_31_19165_s_123	9235906	As shown in Table  II, NKC6 cells producing YOR071c or YOR192c protein showed the thiamin transport activities of 13.7% and 41.0%, respectively, compared with the cells expressing THI10 protein.	gene_phenotype
68915	6	333351	7	NULL	NULL	0	NULL	statement 5	Process		shows					thiamin	Chemical	transport activities of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_31_19165_s_123	9235906	As shown in Table  II, NKC6 cells producing YOR071c or YOR192c protein showed the thiamin transport activities of 13.7% and 41.0%, respectively, compared with the cells expressing THI10 protein.	gene_phenotype
68916	1	333352	7	NULL	NULL	0	NULL	MEI5 YPL121c Meiotic protein	GP		required for					synapsis	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_314	15334557	MEI5   YPL121c Meiotic protein required for synapsis and meiotic recombination	gene_phenotype
68917	2	333352	7	NULL	NULL	0	NULL	MEI5 YPL121c Meiotic protein	GP		required for					meiotic recombination	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_314	15334557	MEI5   YPL121c Meiotic protein required for synapsis and meiotic recombination	gene_phenotype
68918	1	333353	7	NULL	NULL	0	NULL	Ppp4c-R2	GP		is essential for					microtubule-related processes 	GP	centrosomes			NULL	higher eukaryotes	0	NULL	NULL	NULL	abs-batch0740-0759_febs-j_273_14_16857015_s_6	16857015	Despite the essential function of Ppp4c-R2 in microtubule-related  processes at centrosomes in higher eukaryotes, S. cerevisiae diploid strains  with homozygous deletion of YBL046w and two or one functional copies of  the TUB2 gene were viable and no more sensitive to microtubule-depolymerizing  drugs than the control strain.	gene_phenotype
68919	2	333353	7	NULL	NULL	0	NULL	YBL046w	GP	S. cerevisiae;;diploid strains with homozygous deletion of	is					viable	Process				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_febs-j_273_14_16857015_s_6	16857015	Despite the essential function of Ppp4c-R2 in microtubule-related  processes at centrosomes in higher eukaryotes, S. cerevisiae diploid strains  with homozygous deletion of YBL046w and two or one functional copies of  the TUB2 gene were viable and no more sensitive to microtubule-depolymerizing  drugs than the control strain.	gene_phenotype
68920	3	333353	7	NULL	NULL	NULL	NULL	TUB2 gene	GP	S. cerevisiae;;diploid strains with homozygous deletion of 	is 					viable	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_febs-j_273_14_16857015_s_6	16857015	Despite the essential function of Ppp4c-R2 in microtubule-related  processes at centrosomes in higher eukaryotes, S. cerevisiae diploid strains  with homozygous deletion of YBL046w and two or one functional copies of  the TUB2 gene were viable and no more sensitive to microtubule-depolymerizing  drugs than the control strain.	gene_phenotype
68921	4	333353	7	NULL	NULL	NULL	NULL	statement 2	Process		is not sensitive to					microtubule-depolymerizing drugs	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_febs-j_273_14_16857015_s_6	16857015	Despite the essential function of Ppp4c-R2 in microtubule-related  processes at centrosomes in higher eukaryotes, S. cerevisiae diploid strains  with homozygous deletion of YBL046w and two or one functional copies of  the TUB2 gene were viable and no more sensitive to microtubule-depolymerizing  drugs than the control strain.	gene_phenotype
68922	5	333353	7	NULL	NULL	0	NULL	statement 3	Process		is not sensitive to					microtubule-depolymerizing drugs	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_febs-j_273_14_16857015_s_6	16857015	Despite the essential function of Ppp4c-R2 in microtubule-related  processes at centrosomes in higher eukaryotes, S. cerevisiae diploid strains  with homozygous deletion of YBL046w and two or one functional copies of  the TUB2 gene were viable and no more sensitive to microtubule-depolymerizing  drugs than the control strain.	gene_phenotype
68923	1	333355	7	NULL	NULL	0	NULL	Ybr296c protein	GP		is a type of					Na+-coupled phosphate transporter of the plasma membrane	GP	high-affinity			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1422_3_255_s_159	10548719	The strong sequence identity (45%) and similarity (67%) [ 15 and  73] between this gene product and the previously identified Pho-4 phosphate transporter of the related organism  Neurospora crassa [  83] suggested that the Ybr296c protein might be the previously proposed high-affinity Na+-coupled phosphate transporter of the plasma membrane [ 16].	gene_phenotype
68924	1	333356	7	NULL	NULL	NULL	NULL	YDL074C	GP	deletion of	increase					chromosome 	Chromosome	loss of			NULL	haploid strain	NULL	NULL	NULL	NULL	gw60_pnas_97_24_13203_s_108	11087867	Interestingly, however, deletion of the gene encoding one of these proteins (YDL074C), in a haploid strain, results in an approximately 10-fold increase in the rate of chromosome loss (J.R.S.N. and P.S.K., unpublished data), as measured by a colony sectoring assay ( 36).	gene_phenotype
68925	1	333357	7	NULL	NULL	0	NULL	YDR208w PTP2	GP		downregulate					Hog1p	GP	sporulation of			NULL		0	NULL	NULL	NULL	gw70_yeast_19_7_587_s_66	11967829	YDR208w   PTP2 Downregulate Hog1p and Fus3p MAPK, sporulation (James  et al., [ 1992]; Maeda  et al., [ 1994]; Wurgler-Murphy  et al., [ 1997]; Zhan  et al., [ 2000])	gene_phenotype
68926	2	333357	7	NULL	NULL	0	NULL	YDR208w PTP2	GP		downregulate					Fus3p MAPK	GP	sporulation of			NULL		0	NULL	NULL	NULL	gw70_yeast_19_7_587_s_66	11967829	YDR208w   PTP2 Downregulate Hog1p and Fus3p MAPK, sporulation (James  et al., [ 1992]; Maeda  et al., [ 1994]; Wurgler-Murphy  et al., [ 1997]; Zhan  et al., [ 2000])	gene_phenotype
68927	1	333358	7	NULL	NULL	0	NULL	YGR046w	GP	 Saccharomyces cerevisiae 	encode					Mmp37p	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_9_4051_s_27	16790493	We demonstrate that the  Saccharomyces cerevisiae open reading frame (ORF) YGR046w encoding Mmp37p is nonessential for yeast cell viability at 30 degrees C.	gene_phenotype
68928	2	333358	7	NULL	NULL	0	NULL	statement 1	Process		is nonessential for					 yeast cell	Cell	viability of			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_9_4051_s_27	16790493	We demonstrate that the  Saccharomyces cerevisiae open reading frame (ORF) YGR046w encoding Mmp37p is nonessential for yeast cell viability at 30 degrees C.	gene_phenotype
68929	3	333358	7	NULL	NULL	0	NULL	ORF	GP		is 					open reading frame	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_9_4051_s_27	16790493	We demonstrate that the  Saccharomyces cerevisiae open reading frame (ORF) YGR046w encoding Mmp37p is nonessential for yeast cell viability at 30 degrees C.	gene_phenotype
68930	1	333359	7	NULL	NULL	0	NULL	YJR059w	GP		corresponds to					PTK2/STK2	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_20_7654_s_137	11003661	YJR059w corresponds to  PTK2/STK2, the protein kinase gene previously described as being required for polyamine transport ( 26,  36).	gene_phenotype
68931	2	333359	7	NULL	NULL	0	NULL	PTK2/STK2	GP		is a type of					protein kinase gene	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_20_7654_s_137	11003661	YJR059w corresponds to  PTK2/STK2, the protein kinase gene previously described as being required for polyamine transport ( 26,  36).	gene_phenotype
68932	3	333359	7	NULL	NULL	0	NULL	PTK2/STK2	GP		is required for					polyamine transport	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_20_7654_s_137	11003661	YJR059w corresponds to  PTK2/STK2, the protein kinase gene previously described as being required for polyamine transport ( 26,  36).	gene_phenotype
68933	1	333360	7	NULL	NULL	NULL	NULL	Nse5	GP	budding yeast	does not have 					sequence homologues	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_5_1617_s_120	16478984	Nse5 and Nse6, like KRE29 and YML023c in budding yeast, have no sequence homologues in other species.	gene_phenotype
68934	2	333360	7	NULL	NULL	0	NULL	Nse6	GP	budding yeast	does not have					sequence homologue	GP				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_5_1617_s_120	16478984	Nse5 and Nse6, like KRE29 and YML023c in budding yeast, have no sequence homologues in other species.	gene_phenotype
68935	3	333360	7	NULL	NULL	0	NULL	KRE29	GP	budding yeast	does not have					sequence homologues	GP				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_5_1617_s_120	16478984	Nse5 and Nse6, like KRE29 and YML023c in budding yeast, have no sequence homologues in other species.	gene_phenotype
68936	4	333360	7	NULL	NULL	0	NULL	YML023c	GP	budding yeast	does not have					sequence homologues	GP				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_5_1617_s_120	16478984	Nse5 and Nse6, like KRE29 and YML023c in budding yeast, have no sequence homologues in other species.	gene_phenotype
68937	1	333361	7	NULL	NULL	NULL	NULL	KRE29	GP		is homologous to		functionally			Nse5	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_5_1617_s_386	16478984	It is possible that KRE29/YML023c and Nse5/6 are functionally homologous; however; KRE29 and YML023c are both essential for viability, whereas Nse5 and Nse6 are not.	gene_phenotype
68938	2	333361	7	NULL	NULL	NULL	NULL	YML023c	GP		is homologous to		functionally			Nse5	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_5_1617_s_386	16478984	It is possible that KRE29/YML023c and Nse5/6 are functionally homologous; however; KRE29 and YML023c are both essential for viability, whereas Nse5 and Nse6 are not.	gene_phenotype
68939	3	333361	7	NULL	NULL	0	NULL	KRE29	GP		is essential for					viability	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_5_1617_s_386	16478984	It is possible that KRE29/YML023c and Nse5/6 are functionally homologous; however; KRE29 and YML023c are both essential for viability, whereas Nse5 and Nse6 are not.	gene_phenotype
68940	4	333361	7	NULL	NULL	0	NULL	YML023c	GP		is essential for					viability	GP				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_5_1617_s_386	16478984	It is possible that KRE29/YML023c and Nse5/6 are functionally homologous; however; KRE29 and YML023c are both essential for viability, whereas Nse5 and Nse6 are not.	gene_phenotype
68941	5	333361	7	NULL	NULL	0	NULL	Nse5	GP		is not essential for					viability	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_5_1617_s_386	16478984	It is possible that KRE29/YML023c and Nse5/6 are functionally homologous; however; KRE29 and YML023c are both essential for viability, whereas Nse5 and Nse6 are not.	gene_phenotype
68942	6	333361	7	NULL	NULL	0	NULL	Nse6 	GP		is not essential for					viability	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_5_1617_s_386	16478984	It is possible that KRE29/YML023c and Nse5/6 are functionally homologous; however; KRE29 and YML023c are both essential for viability, whereas Nse5 and Nse6 are not.	gene_phenotype
68943	7	333361	7	NULL	NULL	0	NULL	KRE29	GP		is homologous to		functionally			Nse6	GP				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_5_1617_s_386	16478984	It is possible that KRE29/YML023c and Nse5/6 are functionally homologous; however; KRE29 and YML023c are both essential for viability, whereas Nse5 and Nse6 are not.	gene_phenotype
68944	8	333361	7	NULL	NULL	0	NULL	YML023c	GP		is homologous to		functionally			Nse6	GP				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_5_1617_s_386	16478984	It is possible that KRE29/YML023c and Nse5/6 are functionally homologous; however; KRE29 and YML023c are both essential for viability, whereas Nse5 and Nse6 are not.	gene_phenotype
68945	1	333362	7	NULL	NULL	NULL	NULL	SMC5/6 complex	GP	budding yeast	contains					Nse1	GP		well-conserved non-SMC subunits		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_5_1617_s_36	16478984	In addition to the four well-conserved non-SMC subunits (Nse1 to -4), the budding yeast SMC5/6 complex contains two other essential subunits, YML023c and KRE29, which are not conserved at the primary sequence level in other species ( ,  ).	gene_phenotype
68946	2	333362	7	NULL	NULL	0	NULL	SMC5/6 complex	GP	budding yeast	contains					Nse2	GP		well-conserved non-SMC subunits		NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_5_1617_s_36	16478984	In addition to the four well-conserved non-SMC subunits (Nse1 to -4), the budding yeast SMC5/6 complex contains two other essential subunits, YML023c and KRE29, which are not conserved at the primary sequence level in other species ( ,  ).	gene_phenotype
68947	3	333362	7	NULL	NULL	NULL	NULL	SMC5/6 complex	GP	budding yeast	contains					Nse3	GP		well-conserved non-SMC subunits 		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_5_1617_s_36	16478984	In addition to the four well-conserved non-SMC subunits (Nse1 to -4), the budding yeast SMC5/6 complex contains two other essential subunits, YML023c and KRE29, which are not conserved at the primary sequence level in other species ( ,  ).	gene_phenotype
68948	4	333362	7	NULL	NULL	NULL	NULL	SMC5/6 complex 	GP	budding yeast	contains					Nse4	GP		well-conserved non-SMC subunits		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_5_1617_s_36	16478984	In addition to the four well-conserved non-SMC subunits (Nse1 to -4), the budding yeast SMC5/6 complex contains two other essential subunits, YML023c and KRE29, which are not conserved at the primary sequence level in other species ( ,  ).	gene_phenotype
68949	5	333362	7	NULL	NULL	0	NULL	SMC5/6 complex 	GP	budding yeast	contains					YML023c subunits	GP	essential			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_5_1617_s_36	16478984	In addition to the four well-conserved non-SMC subunits (Nse1 to -4), the budding yeast SMC5/6 complex contains two other essential subunits, YML023c and KRE29, which are not conserved at the primary sequence level in other species ( ,  ).	gene_phenotype
68950	6	333362	7	NULL	NULL	0	NULL	SMC5/6 complex	GP	budding yeast	contains					KRE29 subunits	GP	essential			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_5_1617_s_36	16478984	In addition to the four well-conserved non-SMC subunits (Nse1 to -4), the budding yeast SMC5/6 complex contains two other essential subunits, YML023c and KRE29, which are not conserved at the primary sequence level in other species ( ,  ).	gene_phenotype
69095	1	333363	7	NULL	NULL	0	NULL	SIL1 ORF	GP	deltasil1 null mutant	is non-essential for					viability	Process				NULL		0	NULL	NULL	NULL	gw60_embo_19_23_6440_s_136	11101517	Phenotypic analysis of a deltasil1 null mutant   The  SIL1 ORF (YOL031c) was disrupted as part of the Eurofan project and shown to be non-essential for viability.	gene_phenotype
69096	1	333364	7	NULL	NULL	0	NULL	GYP1	GP		is a type of					GTPase activating protein	GP				NULL		0	NULL	NULL	NULL	gw60_science_285_5429_901_s_109	10436161	GYP1 ( YOR070C) is a GTPase activating protein for Sec4p, a protein in the secretion pathway ( 16).	gene_phenotype
69097	2	333364	7	NULL	NULL	0	NULL	GYP1	GP		is					YOR070C	GP				NULL		0	NULL	NULL	NULL	gw60_science_285_5429_901_s_109	10436161	GYP1 ( YOR070C) is a GTPase activating protein for Sec4p, a protein in the secretion pathway ( 16).	gene_phenotype
69098	3	333364	7	NULL	NULL	0	NULL	statement 1	Process		is required for					Sec4p	GP				NULL		0	NULL	NULL	NULL	gw60_science_285_5429_901_s_109	10436161	GYP1 ( YOR070C) is a GTPase activating protein for Sec4p, a protein in the secretion pathway ( 16).	gene_phenotype
69099	4	333364	7	NULL	NULL	0	NULL	Sec4p	GP		is a protein in					secretion pathway	Process				NULL		0	NULL	NULL	NULL	gw60_science_285_5429_901_s_109	10436161	GYP1 ( YOR070C) is a GTPase activating protein for Sec4p, a protein in the secretion pathway ( 16).	gene_phenotype
69100	1	333365	7	NULL	NULL	0	NULL	YPL157W gene 	GP	yeast strain;null mutation	is found to be					viable	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_98_18_10380_s_205	11517327	The yeast strain with null mutation of YPL157W gene has been generated by the  Saccharomyces Genome Deletion Project and has turned out to be viable.	gene_phenotype
69101	1	333366	7	NULL	NULL	0	NULL	YBL051C	GP		designated as					PIN4	GP				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_7_2779_s_207	15024067	In another study,  YBL051C was designated  PIN4 because it is present on a plasmid that can induce prion formation in yeast cells when overexpressed at very high levels ( ).	gene_phenotype
69103	2	333366	7	NULL	NULL	0	NULL	statement 1	Process		induce					prion	GP	formation of			NULL	yeast cells	0	NULL	NULL	NULL	gw70_molcellbiol_24_7_2779_s_207	15024067	In another study,  YBL051C was designated  PIN4 because it is present on a plasmid that can induce prion formation in yeast cells when overexpressed at very high levels ( ).	gene_phenotype
69104	3	333366	7	NULL	NULL	0	NULL	statement 2	Process		occurs when					high levels	Process	overexpressed at			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_7_2779_s_207	15024067	In another study,  YBL051C was designated  PIN4 because it is present on a plasmid that can induce prion formation in yeast cells when overexpressed at very high levels ( ).	gene_phenotype
69105	1	333367	7	NULL	NULL	NULL	NULL	cells 	Cell	S. cerevisiae;;depleted of Ybr004cp	have					cell walls	Cell	weakened			NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_febs-j_272_5_15720390_s_4	15720390	S. cerevisiae cells depleted of Ybr004cp have weakened cell  walls and abnormal morphology, are unable to incorporate [3]inositol  into proteins, and accumulate a GPI intermediate having a single mannose  that is likely modified with ethanolamine phosphate.	gene_phenotype
69106	2	333367	7	NULL	NULL	NULL	NULL	cells	Cell	S. cerevisiae;;depleted of Ybr004cp	have					 morphology	Process	abnormal			NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_febs-j_272_5_15720390_s_4	15720390	S. cerevisiae cells depleted of Ybr004cp have weakened cell  walls and abnormal morphology, are unable to incorporate [3]inositol  into proteins, and accumulate a GPI intermediate having a single mannose  that is likely modified with ethanolamine phosphate.	gene_phenotype
69107	3	333367	7	NULL	NULL	0	NULL	inositol	Chemical		incorporated into					proteins	GP				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_febs-j_272_5_15720390_s_4	15720390	S. cerevisiae cells depleted of Ybr004cp have weakened cell  walls and abnormal morphology, are unable to incorporate [3]inositol  into proteins, and accumulate a GPI intermediate having a single mannose  that is likely modified with ethanolamine phosphate.	gene_phenotype
69108	4	333367	7	NULL	NULL	0	NULL	cells	Cell	S. cerevisiae;;depleted of Ybr004cp	are unable to incorporate					statement 3	Process				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_febs-j_272_5_15720390_s_4	15720390	S. cerevisiae cells depleted of Ybr004cp have weakened cell  walls and abnormal morphology, are unable to incorporate [3]inositol  into proteins, and accumulate a GPI intermediate having a single mannose  that is likely modified with ethanolamine phosphate.	gene_phenotype
69109	5	333367	7	NULL	NULL	0	NULL	GPI intermediate	Chemical	S. cerevisiae;;depleted of Ybr004cp	have					single mannose	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_febs-j_272_5_15720390_s_4	15720390	S. cerevisiae cells depleted of Ybr004cp have weakened cell  walls and abnormal morphology, are unable to incorporate [3]inositol  into proteins, and accumulate a GPI intermediate having a single mannose  that is likely modified with ethanolamine phosphate.	gene_phenotype
69110	6	333367	7	NULL	NULL	0	NULL	GPI intermediate	Chemical	single mannose	is modified with					ethanolamine phosphate	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_febs-j_272_5_15720390_s_4	15720390	S. cerevisiae cells depleted of Ybr004cp have weakened cell  walls and abnormal morphology, are unable to incorporate [3]inositol  into proteins, and accumulate a GPI intermediate having a single mannose  that is likely modified with ethanolamine phosphate.	gene_phenotype
69111	7	333367	7	NULL	NULL	0	NULL	Cells	Cell	S. cerevisiae;;depleted of Ybr004cp	accumulate					GPI intermediate	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_febs-j_272_5_15720390_s_4	15720390	S. cerevisiae cells depleted of Ybr004cp have weakened cell  walls and abnormal morphology, are unable to incorporate [3]inositol  into proteins, and accumulate a GPI intermediate having a single mannose  that is likely modified with ethanolamine phosphate.	gene_phenotype
69112	1	333369	7	NULL	NULL	0	NULL	CSM1	GP		is					chromosome segregation in meiosis	GP				NULL		0	NULL	NULL	NULL	gw60_devcell_4_4_535_s_81	12689592	CSM1 (chromosome segregation in meiosis; ORF YCR086W) has already been shown to have a role in meiotic chromosome segregation  (Rabitsch et al., 2001  ).	gene_phenotype
69113	2	333369	7	NULL	NULL	0	NULL	CSM1	GP		have a role in					meiotic chromosome segregation	Process				NULL		0	NULL	NULL	NULL	gw60_devcell_4_4_535_s_81	12689592	CSM1 (chromosome segregation in meiosis; ORF YCR086W) has already been shown to have a role in meiotic chromosome segregation  (Rabitsch et al., 2001  ).	gene_phenotype
69114	1	333370	7	NULL	NULL	NULL	NULL	Yer010c protein	GP		shares					RraA family	GP	a common fold with proteins of regulators of			NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_protein-sci_14_10_16195557_s_2	16195557	We present here the structure of Yer010c protein of unknown function, solved  by Multiple Anomalous Diffraction and revealing a common fold and oligomerization  state with proteins of the regulator of ribonuclease activity A (RraA)  family.	gene_phenotype
69115	2	333370	7	NULL	NULL	NULL	NULL	Yer010c protein	GP		shares					RraA family	GP	oligomerization state with proteins of regulators of			NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_protein-sci_14_10_16195557_s_2	16195557	We present here the structure of Yer010c protein of unknown function, solved  by Multiple Anomalous Diffraction and revealing a common fold and oligomerization  state with proteins of the regulator of ribonuclease activity A (RraA)  family.	gene_phenotype
69116	3	333370	7	NULL	NULL	0	NULL	RraA	GP		is					ribonuclease activity A 	GP				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_protein-sci_14_10_16195557_s_2	16195557	We present here the structure of Yer010c protein of unknown function, solved  by Multiple Anomalous Diffraction and revealing a common fold and oligomerization  state with proteins of the regulator of ribonuclease activity A (RraA)  family.	gene_phenotype
69117	1	333371	7	NULL	NULL	0	NULL	YHR158c	GP	overexpression of	suppresses		partially			mating defect	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_143_2_375_s_202	9786949	We conclude that overexpression of YHR158c partially suppresses the  mating defect exhibited by a subset of mutants defective in  cell fusion.	gene_phenotype
69118	2	333371	7	NULL	NULL	NULL	NULL	cell fusion	Process	subset of mutants defective in	shows					mating defect	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_143_2_375_s_202	9786949	We conclude that overexpression of YHR158c partially suppresses the  mating defect exhibited by a subset of mutants defective in  cell fusion.	gene_phenotype
69119	1	333372	7	NULL	NULL	0	NULL	ORF YIL019w	GP		is					FAF1	GP				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_319_2_349_s_62	15178413	ORF  YIL019w ( FAF1) encodes a protein of 346 amino acids essential for cell viability.	gene_phenotype
69120	2	333372	7	NULL	NULL	0	NULL	FAF1	GP		encode					 protein of 346 amino acids 	GP				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_319_2_349_s_62	15178413	ORF  YIL019w ( FAF1) encodes a protein of 346 amino acids essential for cell viability.	gene_phenotype
69121	3	333372	7	NULL	NULL	0	NULL	statement 1	GP		essential for					cell viability	Process				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_319_2_349_s_62	15178413	ORF  YIL019w ( FAF1) encodes a protein of 346 amino acids essential for cell viability.	gene_phenotype
69122	1	333373	7	NULL	NULL	0	NULL	YLL060C	GP	protein product of	activates					GST	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_45_29915_s_125	9792709	Again, after we had confirmed that the protein product of YLL060C exhibits GST activity (described below), we named it  GTT2 ( gluta thione  transferase  2).	gene_phenotype
69123	2	333373	7	NULL	NULL	0	NULL	YLL060C	GP	protein product of	is					GTT2	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_45_29915_s_125	9792709	Again, after we had confirmed that the protein product of YLL060C exhibits GST activity (described below), we named it  GTT2 ( gluta thione  transferase  2).	gene_phenotype
69124	3	333373	7	NULL	NULL	0	NULL	GTT2	GP		is					gluta thione transferase 2	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_45_29915_s_125	9792709	Again, after we had confirmed that the protein product of YLL060C exhibits GST activity (described below), we named it  GTT2 ( gluta thione  transferase  2).	gene_phenotype
69125	1	333375	7	NULL	NULL	0	NULL	YLR226w	GP		encode					BUR2	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_19_7080_s_113	10982824	These results indicate that YLR226w encodes  BUR2, that  BUR2 is not essential for viability but is important for normal growth, and that loss of function causes the Bur  phenotype.	gene_phenotype
69126	2	333375	7	NULL	NULL	0	NULL	BUR2	GP		is not essential for					viability 	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_19_7080_s_113	10982824	These results indicate that YLR226w encodes  BUR2, that  BUR2 is not essential for viability but is important for normal growth, and that loss of function causes the Bur  phenotype.	gene_phenotype
69127	3	333375	7	NULL	NULL	0	NULL	BUR2	GP		is important for					normal growth	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_19_7080_s_113	10982824	These results indicate that YLR226w encodes  BUR2, that  BUR2 is not essential for viability but is important for normal growth, and that loss of function causes the Bur  phenotype.	gene_phenotype
69128	4	333375	7	NULL	NULL	0	NULL	function	Process	loss of	cause					Bur phenotype	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_19_7080_s_113	10982824	These results indicate that YLR226w encodes  BUR2, that  BUR2 is not essential for viability but is important for normal growth, and that loss of function causes the Bur  phenotype.	gene_phenotype
69129	1	333376	7	NULL	NULL	0	NULL	YLR285W	GP	manipulation of	affects					lifespan	Process				NULL		0	NULL	NULL	NULL	gw70_nature_423_6936_181_s_107	12736687	e, Manipulation of YLR285W affects lifespan.	gene_phenotype
69130	1	333377	7	NULL	NULL	0	NULL	YLR285W	GP		increase					lifespan	Process	yeast			NULL		0	NULL	NULL	NULL	gw70_nature_423_6936_181_s_122	12736687	Additional copies of YLR285W increased yeast lifespan and this effect was not enhanced  by glucose restriction ( Fig. 4e).	gene_phenotype
69131	2	333377	7	NULL	NULL	0	NULL	glucose	Chemical	restriction of	does not enhance					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_nature_423_6936_181_s_122	12736687	Additional copies of YLR285W increased yeast lifespan and this effect was not enhanced  by glucose restriction ( Fig. 4e).	gene_phenotype
69132	1	333378	7	NULL	NULL	0	NULL	YLR285W	GP		increase					silencing	Process				NULL		0	NULL	NULL	NULL	gw70_nature_423_6936_181_s_121	12736687	Additional copies of YLR285W increased silencing, whereas deletion of this gene  led to a loss of silencing, similar to the effect of manipulating  PNC1 (ref.  16) ( Fig. 4d).	gene_phenotype
69133	2	333378	7	NULL	NULL	0	NULL	YLR285W gene	GP	deletion of	leads to					silencing	Process	loss of			NULL		0	NULL	NULL	NULL	gw70_nature_423_6936_181_s_121	12736687	Additional copies of YLR285W increased silencing, whereas deletion of this gene  led to a loss of silencing, similar to the effect of manipulating  PNC1 (ref.  16) ( Fig. 4d).	gene_phenotype
69134	3	333378	7	NULL	NULL	0	NULL	statement 2	Process		similar to					PNC1	GP	effect of manipulating			NULL		0	NULL	NULL	NULL	gw70_nature_423_6936_181_s_121	12736687	Additional copies of YLR285W increased silencing, whereas deletion of this gene  led to a loss of silencing, similar to the effect of manipulating  PNC1 (ref.  16) ( Fig. 4d).	gene_phenotype
69135	1	333379	7	NULL	NULL	0	NULL	YLR285W	GP		is not a true					longevity regulator	Process				NULL		0	NULL	NULL	NULL	gw70_nature_423_6936_181_s_123	12736687	Unlike  PNC1, YLR285W is not a true longevity regulator because its expression is not apparently  modulated by stimuli that extend lifespan 18, and its deletion does not abolish lifespan extension by glucose restriction ( Fig. 4e).	gene_phenotype
69136	2	333379	7	NULL	NULL	0	NULL	YLR285W	GP		is not like					PNC1	GP				NULL		0	NULL	NULL	NULL	gw70_nature_423_6936_181_s_123	12736687	Unlike  PNC1, YLR285W is not a true longevity regulator because its expression is not apparently  modulated by stimuli that extend lifespan 18, and its deletion does not abolish lifespan extension by glucose restriction ( Fig. 4e).	gene_phenotype
69137	3	333379	7	NULL	NULL	0	NULL	YLR285W	GP	expression of	 not modulated by		apparently			lifespan	Process	stimuli extending			NULL		0	NULL	NULL	NULL	gw70_nature_423_6936_181_s_123	12736687	Unlike  PNC1, YLR285W is not a true longevity regulator because its expression is not apparently  modulated by stimuli that extend lifespan 18, and its deletion does not abolish lifespan extension by glucose restriction ( Fig. 4e).	gene_phenotype
69138	4	333379	7	NULL	NULL	0	NULL	lifespan	Process		extend by					glucose	Chemical	restriction of			NULL		0	NULL	NULL	NULL	gw70_nature_423_6936_181_s_123	12736687	Unlike  PNC1, YLR285W is not a true longevity regulator because its expression is not apparently  modulated by stimuli that extend lifespan 18, and its deletion does not abolish lifespan extension by glucose restriction ( Fig. 4e).	gene_phenotype
69139	5	333379	7	NULL	NULL	0	NULL	YLR285W	GP	deletion of	does not abolish					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_nature_423_6936_181_s_123	12736687	Unlike  PNC1, YLR285W is not a true longevity regulator because its expression is not apparently  modulated by stimuli that extend lifespan 18, and its deletion does not abolish lifespan extension by glucose restriction ( Fig. 4e).	gene_phenotype
69140	1	333381	7	NULL	NULL	0	NULL	NPL6 YMR091c 	GP		is a type of					nuclear protein	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_202	15334557	NPL6   YMR091c Nuclear protein, possible role in nuclear protein import	gene_phenotype
69141	2	333381	7	NULL	NULL	0	NULL	statement 1	GP		role in		possible			nuclear protein	GP	import of			NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_202	15334557	NPL6   YMR091c Nuclear protein, possible role in nuclear protein import	gene_phenotype
69142	1	333383	7	NULL	NULL	NULL	NULL	IST2 mRNA	NucleicAcid		localize				RNA motifs from	bud tip	CellComponent	reporter mRNA to			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_11_4752_s_311	15899876	As shown in Fig.  7D, the RNA motifs from the  IST2 and  YMR171c mRNAs were able to localize a reporter mRNA to the bud tip, suggesting that both act as functional localization elements.	gene_phenotype
69143	2	333383	7	NULL	NULL	NULL	NULL	YMR171c mRNA	NucleicAcid		localize				RNA motifs from	bud tip	CellComponent	reporter mRNA to			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_11_4752_s_311	15899876	As shown in Fig.  7D, the RNA motifs from the  IST2 and  YMR171c mRNAs were able to localize a reporter mRNA to the bud tip, suggesting that both act as functional localization elements.	gene_phenotype
69144	3	333383	7	NULL	NULL	0	NULL	IST2 mRNA	NucleicAcid		act as					 functional localization elements	GP				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_11_4752_s_311	15899876	As shown in Fig.  7D, the RNA motifs from the  IST2 and  YMR171c mRNAs were able to localize a reporter mRNA to the bud tip, suggesting that both act as functional localization elements.	gene_phenotype
69145	4	333383	7	NULL	NULL	NULL	NULL	YMR171c mRNA	NucleicAcid		act as 					 functional localization elements	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_11_4752_s_311	15899876	As shown in Fig.  7D, the RNA motifs from the  IST2 and  YMR171c mRNAs were able to localize a reporter mRNA to the bud tip, suggesting that both act as functional localization elements.	gene_phenotype
69146	5	333383	7	NULL	NULL	0	NULL	statement 1	Process		suggest					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_11_4752_s_311	15899876	As shown in Fig.  7D, the RNA motifs from the  IST2 and  YMR171c mRNAs were able to localize a reporter mRNA to the bud tip, suggesting that both act as functional localization elements.	gene_phenotype
69147	6	333383	7	NULL	NULL	0	NULL	statement 2	Process		suggest					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_11_4752_s_311	15899876	As shown in Fig.  7D, the RNA motifs from the  IST2 and  YMR171c mRNAs were able to localize a reporter mRNA to the bud tip, suggesting that both act as functional localization elements.	gene_phenotype
69148	1	333384	7	NULL	NULL	NULL	NULL	She2p	GP		recognize					 ASH1 mRNA	NucleicAcid	bud-localized		RNA motif in the localization elements of	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_11_4752_s_340	15899876	The identification of the same RNA motif in the localization elements of the bud-localized  ASH1,  IST2, and  YMR171c mRNAs strongly supports our conclusion that this motif contains the main determinants required for their recognition by She2p.	gene_phenotype
69149	2	333384	7	NULL	NULL	0	NULL	She2p	GP		recognize					 IST2 mRNA	NucleicAcid	bud-localized		RNA motif in the localization elements of	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_11_4752_s_340	15899876	The identification of the same RNA motif in the localization elements of the bud-localized  ASH1,  IST2, and  YMR171c mRNAs strongly supports our conclusion that this motif contains the main determinants required for their recognition by She2p.	gene_phenotype
69150	3	333384	7	NULL	NULL	0	NULL	She2p	GP		recognize					YMR171c mRNA	NucleicAcid	bud-localized		RNA motif in the localization elements of	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_11_4752_s_340	15899876	The identification of the same RNA motif in the localization elements of the bud-localized  ASH1,  IST2, and  YMR171c mRNAs strongly supports our conclusion that this motif contains the main determinants required for their recognition by She2p.	gene_phenotype
69151	1	333385	7	NULL	NULL	0	NULL	YOR129c	GP	S.cerevisiae	is not required for					viability	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_8_3658_s_283	15155805	In  S. cerevisiae, YOR129c is not required for viability (Winzeler  et al., 1999 ), but the observation that its expression is induced by mating pheromone in a Ste12p-dependent manner suggests that it may play a role in mating (Ren  et al., 2000 ).	gene_phenotype
69152	2	333385	7	NULL	NULL	0	NULL	YOR129c	GP	expression of	induced by					mating pheromone	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_8_3658_s_283	15155805	In  S. cerevisiae, YOR129c is not required for viability (Winzeler  et al., 1999 ), but the observation that its expression is induced by mating pheromone in a Ste12p-dependent manner suggests that it may play a role in mating (Ren  et al., 2000 ).	gene_phenotype
69153	3	333385	7	NULL	NULL	0	NULL	statement 2	Process		depends on					Ste12p	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_8_3658_s_283	15155805	In  S. cerevisiae, YOR129c is not required for viability (Winzeler  et al., 1999 ), but the observation that its expression is induced by mating pheromone in a Ste12p-dependent manner suggests that it may play a role in mating (Ren  et al., 2000 ).	gene_phenotype
69154	4	333385	7	NULL	NULL	0	NULL	YOR129c	GP		play a role in		may			mating	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_8_3658_s_283	15155805	In  S. cerevisiae, YOR129c is not required for viability (Winzeler  et al., 1999 ), but the observation that its expression is induced by mating pheromone in a Ste12p-dependent manner suggests that it may play a role in mating (Ren  et al., 2000 ).	gene_phenotype
69155	1	333386	7	NULL	NULL	0	NULL	yor129c	GP	mutant	displays					mating projections	CellComponent	no defects in formation of			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_8_3658_s_382	15155805	However, in both unilateral and bilateral mutant crosses,  yor129c mutants displayed no obvious defects in the formation of mating projections, in cell fusion, or in mating efficiency (our unpublished results).	gene_phenotype
69156	2	333386	7	NULL	NULL	0	NULL	yor129c	GP	mutant	displays					cell fusion	Process	no defects in			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_8_3658_s_382	15155805	However, in both unilateral and bilateral mutant crosses,  yor129c mutants displayed no obvious defects in the formation of mating projections, in cell fusion, or in mating efficiency (our unpublished results).	gene_phenotype
69157	3	333386	7	NULL	NULL	0	NULL	yor129c	GP	mutant	displays					mating efficiency	Process	no defects in			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_8_3658_s_382	15155805	However, in both unilateral and bilateral mutant crosses,  yor129c mutants displayed no obvious defects in the formation of mating projections, in cell fusion, or in mating efficiency (our unpublished results).	gene_phenotype
69158	1	333387	7	NULL	NULL	0	NULL	Yor284w-YFP fusion	GP		localized to					mobile punctate structures 	CellComponent				NULL	cell	0	NULL	NULL	NULL	gw60_cellbiol_154_3_549_s_317	11489916	The Yor284w-YFP fusion localized to a few distinct, mobile punctate structures in the cell (Figs. 4, M and  N and 6, A and  B).	gene_phenotype
69159	1	333388	7	NULL	NULL	0	NULL	Budding yeast	Organism		contains					Mpt5/Uth4	GP		conserved Puf motif		NULL		0	NULL	NULL	NULL	gw60_embo_20_3_552_s_4	11157761	Budding yeast,  Saccharomyces cerevisiae, has five proteins with conserved Puf motifs: Mpt5/Uth4, Ygl014w, Yll013c, Jsn1 and Ypr042c.	gene_phenotype
69160	2	333388	7	NULL	NULL	0	NULL	Budding yeast	Organism		contains					Ygl014w	GP		conserved Puf motif		NULL		0	NULL	NULL	NULL	gw60_embo_20_3_552_s_4	11157761	Budding yeast,  Saccharomyces cerevisiae, has five proteins with conserved Puf motifs: Mpt5/Uth4, Ygl014w, Yll013c, Jsn1 and Ypr042c.	gene_phenotype
69161	3	333388	7	NULL	NULL	0	NULL	Budding yeast	Organism		contains					Yll013c	GP		conserved Puf motif		NULL		0	NULL	NULL	NULL	gw60_embo_20_3_552_s_4	11157761	Budding yeast,  Saccharomyces cerevisiae, has five proteins with conserved Puf motifs: Mpt5/Uth4, Ygl014w, Yll013c, Jsn1 and Ypr042c.	gene_phenotype
69162	4	333388	7	NULL	NULL	0	NULL	Budding yeast	Organism		contains					Jsn1	GP		conserved Puf motif		NULL		0	NULL	NULL	NULL	gw60_embo_20_3_552_s_4	11157761	Budding yeast,  Saccharomyces cerevisiae, has five proteins with conserved Puf motifs: Mpt5/Uth4, Ygl014w, Yll013c, Jsn1 and Ypr042c.	gene_phenotype
69163	5	333388	7	NULL	NULL	NULL	NULL	Budding yeast	Organism		contains					Ypr042c	GP		conserved Puf motif		NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_552_s_4	11157761	Budding yeast,  Saccharomyces cerevisiae, has five proteins with conserved Puf motifs: Mpt5/Uth4, Ygl014w, Yll013c, Jsn1 and Ypr042c.	gene_phenotype
69164	6	333388	7	NULL	NULL	0	NULL	Saccharomyces cerevisiae	Organism		contains					Mpt5/Uth4	GP		conserved Puf motif		NULL		0	NULL	NULL	NULL	gw60_embo_20_3_552_s_4	11157761	Budding yeast,  Saccharomyces cerevisiae, has five proteins with conserved Puf motifs: Mpt5/Uth4, Ygl014w, Yll013c, Jsn1 and Ypr042c.	gene_phenotype
69165	7	333388	7	NULL	NULL	0	NULL	Saccharomyces cerevisiae	Organism		contains					Ygl014w	GP		conserved Puf motif		NULL		0	NULL	NULL	NULL	gw60_embo_20_3_552_s_4	11157761	Budding yeast,  Saccharomyces cerevisiae, has five proteins with conserved Puf motifs: Mpt5/Uth4, Ygl014w, Yll013c, Jsn1 and Ypr042c.	gene_phenotype
69166	8	333388	7	NULL	NULL	0	NULL	Saccharomyces cerevisiae	Organism		contains					Yll013c	GP		conserved Puf motif		NULL		0	NULL	NULL	NULL	gw60_embo_20_3_552_s_4	11157761	Budding yeast,  Saccharomyces cerevisiae, has five proteins with conserved Puf motifs: Mpt5/Uth4, Ygl014w, Yll013c, Jsn1 and Ypr042c.	gene_phenotype
69167	9	333388	7	NULL	NULL	0	NULL	 Saccharomyces cerevisiae	Organism		contains					Jsn1	GP		conserved Puf motif		NULL		0	NULL	NULL	NULL	gw60_embo_20_3_552_s_4	11157761	Budding yeast,  Saccharomyces cerevisiae, has five proteins with conserved Puf motifs: Mpt5/Uth4, Ygl014w, Yll013c, Jsn1 and Ypr042c.	gene_phenotype
69168	10	333388	7	NULL	NULL	0	NULL	 Saccharomyces cerevisiae	Organism		contains					Ypr042c	GP		conserved Puf motif		NULL		0	NULL	NULL	NULL	gw60_embo_20_3_552_s_4	11157761	Budding yeast,  Saccharomyces cerevisiae, has five proteins with conserved Puf motifs: Mpt5/Uth4, Ygl014w, Yll013c, Jsn1 and Ypr042c.	gene_phenotype
69248	1	333389	7	NULL	NULL	NULL	NULL	YPR042C	GP	null mutants	display					viability 	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_552_s_30	11157761	YPR042C null mutants are viable and display increased resistance to cycloheximide and paramomycin, both of which inhibit translation ( Waskiewicz   et al., 1998).	gene_phenotype
69249	2	333389	7	NULL	NULL	0	NULL	statement 1	Process		display					cycloheximide	Chemical	increased resistance to			NULL		0	NULL	NULL	NULL	gw60_embo_20_3_552_s_30	11157761	YPR042C null mutants are viable and display increased resistance to cycloheximide and paramomycin, both of which inhibit translation ( Waskiewicz   et al., 1998).	gene_phenotype
69250	3	333389	7	NULL	NULL	0	NULL	statement 1	Process		display					paramomycin	Chemical	increased resistance to			NULL		0	NULL	NULL	NULL	gw60_embo_20_3_552_s_30	11157761	YPR042C null mutants are viable and display increased resistance to cycloheximide and paramomycin, both of which inhibit translation ( Waskiewicz   et al., 1998).	gene_phenotype
69251	4	333389	7	NULL	NULL	0	NULL	cycloheximide	Chemical		inhibit					translation 	Process				NULL		0	NULL	NULL	NULL	gw60_embo_20_3_552_s_30	11157761	YPR042C null mutants are viable and display increased resistance to cycloheximide and paramomycin, both of which inhibit translation ( Waskiewicz   et al., 1998).	gene_phenotype
69252	5	333389	7	NULL	NULL	NULL	NULL	paramomycin	Chemical		inhibit					translation	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_552_s_30	11157761	YPR042C null mutants are viable and display increased resistance to cycloheximide and paramomycin, both of which inhibit translation ( Waskiewicz   et al., 1998).	gene_phenotype
69253	1	333390	7	NULL	NULL	NULL	NULL	 budding yeast	Organism		contains					Mpt5	GP		three to eight Puf repeats		NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_552_s_24	11157761	The budding yeast,  Saccharomyces cerevisiae, has five proteins that contain three to eight Puf repeats: Mpt5, Ygl014w, Yll013c, Jsn1 and Ypr042c ( Zhang  et al., 1997).	gene_phenotype
69254	2	333390	7	NULL	NULL	0	NULL	 budding yeast	Organism		contains					Ygl014w	GP		three to eight Puf repeats		NULL		0	NULL	NULL	NULL	gw60_embo_20_3_552_s_24	11157761	The budding yeast,  Saccharomyces cerevisiae, has five proteins that contain three to eight Puf repeats: Mpt5, Ygl014w, Yll013c, Jsn1 and Ypr042c ( Zhang  et al., 1997).	gene_phenotype
69255	3	333390	7	NULL	NULL	0	NULL	budding yeast	Organism		contains					Yll013c	GP		three to eight Puf repeats		NULL		0	NULL	NULL	NULL	gw60_embo_20_3_552_s_24	11157761	The budding yeast,  Saccharomyces cerevisiae, has five proteins that contain three to eight Puf repeats: Mpt5, Ygl014w, Yll013c, Jsn1 and Ypr042c ( Zhang  et al., 1997).	gene_phenotype
69256	4	333390	7	NULL	NULL	0	NULL	budding yeast	Organism		contains					Jsn1	GP		three to eight Puf repeats		NULL		0	NULL	NULL	NULL	gw60_embo_20_3_552_s_24	11157761	The budding yeast,  Saccharomyces cerevisiae, has five proteins that contain three to eight Puf repeats: Mpt5, Ygl014w, Yll013c, Jsn1 and Ypr042c ( Zhang  et al., 1997).	gene_phenotype
69257	5	333390	7	NULL	NULL	0	NULL	budding yeast	Organism		contains					Ypr042c	GP		three to eight Puf repeats		NULL		0	NULL	NULL	NULL	gw60_embo_20_3_552_s_24	11157761	The budding yeast,  Saccharomyces cerevisiae, has five proteins that contain three to eight Puf repeats: Mpt5, Ygl014w, Yll013c, Jsn1 and Ypr042c ( Zhang  et al., 1997).	gene_phenotype
69258	6	333390	7	NULL	NULL	0	NULL	Saccharomyces cerevisiae	Organism		contains					Mpt5	GP		three to eight Puf repeats		NULL		0	NULL	NULL	NULL	gw60_embo_20_3_552_s_24	11157761	The budding yeast,  Saccharomyces cerevisiae, has five proteins that contain three to eight Puf repeats: Mpt5, Ygl014w, Yll013c, Jsn1 and Ypr042c ( Zhang  et al., 1997).	gene_phenotype
69259	7	333390	7	NULL	NULL	0	NULL	Saccharomyces cerevisiae	Organism		contains					Ygl014w	GP		three to eight Puf repeats		NULL		0	NULL	NULL	NULL	gw60_embo_20_3_552_s_24	11157761	The budding yeast,  Saccharomyces cerevisiae, has five proteins that contain three to eight Puf repeats: Mpt5, Ygl014w, Yll013c, Jsn1 and Ypr042c ( Zhang  et al., 1997).	gene_phenotype
69260	8	333390	7	NULL	NULL	0	NULL	Saccharomyces cerevisiae	Organism		contains					Yll013c	GP		three to eight Puf repeats		NULL		0	NULL	NULL	NULL	gw60_embo_20_3_552_s_24	11157761	The budding yeast,  Saccharomyces cerevisiae, has five proteins that contain three to eight Puf repeats: Mpt5, Ygl014w, Yll013c, Jsn1 and Ypr042c ( Zhang  et al., 1997).	gene_phenotype
69261	9	333390	7	NULL	NULL	0	NULL	Saccharomyces cerevisiae	Organism		contains only					Jsn1	GP		three to eight Puf repeats		NULL		0	NULL	NULL	NULL	gw60_embo_20_3_552_s_24	11157761	The budding yeast,  Saccharomyces cerevisiae, has five proteins that contain three to eight Puf repeats: Mpt5, Ygl014w, Yll013c, Jsn1 and Ypr042c ( Zhang  et al., 1997).	gene_phenotype
69262	10	333390	7	NULL	NULL	NULL	NULL	Saccharomyces cerevisiae	Organism		contains					Ypr042c	GP		three to eight Puf repeats		NULL		NULL	NULL	NULL	NULL	gw60_embo_20_3_552_s_24	11157761	The budding yeast,  Saccharomyces cerevisiae, has five proteins that contain three to eight Puf repeats: Mpt5, Ygl014w, Yll013c, Jsn1 and Ypr042c ( Zhang  et al., 1997).	gene_phenotype
69263	1	333391	7	NULL	NULL	0	NULL	YPR094w	GP		is required for					cell viability	Process				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_293_2_816_s_239	12054543	To date the molecular and biological functions of  YPR094w is unknown but the systematic deletion of  YPR094w is lethal [  23], pointing out that the protein is required for cell viability.	gene_phenotype
69264	2	333391	7	NULL	NULL	0	NULL	YPR094w	GP	systematic deletion of	is lethal to					cell	Cell				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_293_2_816_s_239	12054543	To date the molecular and biological functions of  YPR094w is unknown but the systematic deletion of  YPR094w is lethal [  23], pointing out that the protein is required for cell viability.	gene_phenotype
69266	1	333393	7	NULL	NULL	0	NULL	 Kar9 protein	GP		play a role in					mitotic spindle	Chromosome	orienting the			NULL	budding yeast	0	NULL	NULL	NULL	gw60_cellbiol_161_3_483_s_177	12743102	The role of the proteins Kar9 and Myo2 in orienting the mitotic spindle of budding yeast.	gene_phenotype
69267	2	333393	7	NULL	NULL	NULL	NULL	Myo2 protein	GP		play a role in					mitotic spindle	Chromosome	orienting the			NULL	budding yeast	NULL	NULL	NULL	NULL	gw60_cellbiol_161_3_483_s_177	12743102	The role of the proteins Kar9 and Myo2 in orienting the mitotic spindle of budding yeast.	gene_phenotype
69268	1	333394	7	NULL	NULL	0	NULL	 YKR087c	GP	yeast	encode					Oma1 	GP	yeast			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46414_s_191	12963738	For reasons outlined below, the yeast protein encoded by YKR087c was termed Oma1 (for overlapping activity with  m-AAA protease).	gene_phenotype
69269	2	333394	7	NULL	NULL	0	NULL	Oma1 	GP		is					overlapping activity with m-AAA protease	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46414_s_191	12963738	For reasons outlined below, the yeast protein encoded by YKR087c was termed Oma1 (for overlapping activity with  m-AAA protease).	gene_phenotype
69270	1	333395	7	NULL	NULL	0	NULL	ylr328w	GP	mutant	display					viability	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_160_3_877_s_360	11901108	Since  ylr328w mutants are viable ( W INZELER et al. 1999   ), the Ygr010w protein likely provides a redundant function.	gene_phenotype
69271	1	333396	7	NULL	NULL	0	NULL	KRI1 	GP	budding yeast	is					KRR1-interacting protein	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_21_7971_s_28	11027267	Here we report the characterization of  KRR1 and a novel  KRI1 (KRR1-interacting protein; YNL308c) gene of budding yeast cells.	gene_phenotype
69272	1	333399	7	NULL	NULL	0	NULL	Munc13 protein	GP		is involved in					vesicle	CellComponent	priming of			NULL		0	NULL	NULL	NULL	gw70_genetics_173_1_49_s_257	16489217	Interestingly, two proteins in this family,  S. pombe SPAC11E3.02c and  S. cerevisiae Yor296w, were previously cited in a study identifying a family of proteins related to the Munc13 protein, which is involved in vesicle priming for neurotransmitter secretion ( OCH et al.).	gene_phenotype
69273	2	333399	7	NULL	NULL	0	NULL	statement 1	Process		required for					neurotransmitter	GP	secretion of			NULL		0	NULL	NULL	NULL	gw70_genetics_173_1_49_s_257	16489217	Interestingly, two proteins in this family,  S. pombe SPAC11E3.02c and  S. cerevisiae Yor296w, were previously cited in a study identifying a family of proteins related to the Munc13 protein, which is involved in vesicle priming for neurotransmitter secretion ( OCH et al.).	gene_phenotype
69274	1	333400	7	NULL	NULL	NULL	NULL	Ypl113cp	GP		activates					hydroxyglutarate dehydrogenase	GP				NULL	S. cerevisiae	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_12_10264_s_35	12525494	Other proteins with homology to Ser3/33p may also be candidates for having hydroxyglutarate  dehydrogenase activity in  S. cerevisiae: (i) Ypl113cp (27% identity), (ii) Ygl185cp (21-23% identity), with similarities to hydroxyacid dehydrogenases, (iii) Fdh1p (26-27% identity), a formate dehydrogenase, and (iv) Ynl274cp (25-26% identity), which is a putative hydroxyisocaproate dehydrogenase ( ).	gene_phenotype
69275	2	333400	7	NULL	NULL	0	NULL	Ygl185cp	GP		is similar to					hydroxyacid dehydrogenases	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10264_s_35	12525494	Other proteins with homology to Ser3/33p may also be candidates for having hydroxyglutarate  dehydrogenase activity in  S. cerevisiae: (i) Ypl113cp (27% identity), (ii) Ygl185cp (21-23% identity), with similarities to hydroxyacid dehydrogenases, (iii) Fdh1p (26-27% identity), a formate dehydrogenase, and (iv) Ynl274cp (25-26% identity), which is a putative hydroxyisocaproate dehydrogenase ( ).	gene_phenotype
69276	3	333400	7	NULL	NULL	0	NULL	Fdh1p	GP		is a type of					formate dehydrogenase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10264_s_35	12525494	Other proteins with homology to Ser3/33p may also be candidates for having hydroxyglutarate  dehydrogenase activity in  S. cerevisiae: (i) Ypl113cp (27% identity), (ii) Ygl185cp (21-23% identity), with similarities to hydroxyacid dehydrogenases, (iii) Fdh1p (26-27% identity), a formate dehydrogenase, and (iv) Ynl274cp (25-26% identity), which is a putative hydroxyisocaproate dehydrogenase ( ).	gene_phenotype
69277	4	333400	7	NULL	NULL	0	NULL	Ynl274cp	GP		is a type of					putative hydroxyisocaproate dehydrogenase 	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10264_s_35	12525494	Other proteins with homology to Ser3/33p may also be candidates for having hydroxyglutarate  dehydrogenase activity in  S. cerevisiae: (i) Ypl113cp (27% identity), (ii) Ygl185cp (21-23% identity), with similarities to hydroxyacid dehydrogenases, (iii) Fdh1p (26-27% identity), a formate dehydrogenase, and (iv) Ynl274cp (25-26% identity), which is a putative hydroxyisocaproate dehydrogenase ( ).	gene_phenotype
69278	5	333400	7	NULL	NULL	0	NULL	Ser3/33p	GP		activates					hydroxyglutarate dehydrogenase 	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10264_s_35	12525494	Other proteins with homology to Ser3/33p may also be candidates for having hydroxyglutarate  dehydrogenase activity in  S. cerevisiae: (i) Ypl113cp (27% identity), (ii) Ygl185cp (21-23% identity), with similarities to hydroxyacid dehydrogenases, (iii) Fdh1p (26-27% identity), a formate dehydrogenase, and (iv) Ynl274cp (25-26% identity), which is a putative hydroxyisocaproate dehydrogenase ( ).	gene_phenotype
69279	1	333403	7	NULL	NULL	0	NULL	histidine	AminoAcid		transported into					vacuoles	CellComponent				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_6_4851_s_94	15572352	Uptake Activities of VBA2 (delta ybr293w) and VBA3 (delta ycl069w) Mutant Vacuolar Membrane Vesicles -- VBA2 ( YBR293w) and  VBA3 ( YCL069w) mutants ( Fig. 4) express candidate genes for histidine transport into vacuoles ( Fig. 1 B), so we measured uptake activities of vacuolar membrane vesicles from these cells.	gene_phenotype
69280	2	333403	7	NULL	NULL	NULL	NULL	VBA2	GP	mutant	express					candidate genes	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_6_4851_s_94	15572352	Uptake Activities of VBA2 (delta ybr293w) and VBA3 (delta ycl069w) Mutant Vacuolar Membrane Vesicles -- VBA2 ( YBR293w) and  VBA3 ( YCL069w) mutants ( Fig. 4) express candidate genes for histidine transport into vacuoles ( Fig. 1 B), so we measured uptake activities of vacuolar membrane vesicles from these cells.	gene_phenotype
69281	3	333403	7	NULL	NULL	0	NULL	VBA3	GP	mutant	express					candidate genes	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_6_4851_s_94	15572352	Uptake Activities of VBA2 (delta ybr293w) and VBA3 (delta ycl069w) Mutant Vacuolar Membrane Vesicles -- VBA2 ( YBR293w) and  VBA3 ( YCL069w) mutants ( Fig. 4) express candidate genes for histidine transport into vacuoles ( Fig. 1 B), so we measured uptake activities of vacuolar membrane vesicles from these cells.	gene_phenotype
69282	4	333403	7	NULL	NULL	0	NULL	statement 2	Process		required for					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_6_4851_s_94	15572352	Uptake Activities of VBA2 (delta ybr293w) and VBA3 (delta ycl069w) Mutant Vacuolar Membrane Vesicles -- VBA2 ( YBR293w) and  VBA3 ( YCL069w) mutants ( Fig. 4) express candidate genes for histidine transport into vacuoles ( Fig. 1 B), so we measured uptake activities of vacuolar membrane vesicles from these cells.	gene_phenotype
69283	5	333403	7	NULL	NULL	0	NULL	statement 3	Process		required for					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_6_4851_s_94	15572352	Uptake Activities of VBA2 (delta ybr293w) and VBA3 (delta ycl069w) Mutant Vacuolar Membrane Vesicles -- VBA2 ( YBR293w) and  VBA3 ( YCL069w) mutants ( Fig. 4) express candidate genes for histidine transport into vacuoles ( Fig. 1 B), so we measured uptake activities of vacuolar membrane vesicles from these cells.	gene_phenotype
69284	1	333404	7	NULL	NULL	0	NULL	fnx1	GP	substrate specificity of	is similar to					 ATR1/SNQ1	GP	budding yeast			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_9_5239_s_197	9710608	The substrate specificity of fnx1 is similar to that of ATR1/SNQ1 from budding yeast; however, the amino acid sequence of ATR1/SNQ1 is not as similar to that of fnx1 as the sequence of the yet uncharacterized  S. cerevisiae ORF ybr293w (Fig.  4A).	gene_phenotype
69285	2	333404	7	NULL	NULL	NULL	NULL	ATR1/SNQ1	GP	amino acid sequence of 	is not similar to					fnx1	GP	amino acid sequence of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5239_s_197	9710608	The substrate specificity of fnx1 is similar to that of ATR1/SNQ1 from budding yeast; however, the amino acid sequence of ATR1/SNQ1 is not as similar to that of fnx1 as the sequence of the yet uncharacterized  S. cerevisiae ORF ybr293w (Fig.  4A).	gene_phenotype
69286	1	333405	7	NULL	NULL	NULL	NULL	 tcrC gene product	GP	Streptomyces aureofaciens	required for					tetracycline	Chemical	resistance to			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_9_5239_s_172	9710608	Figure  4A shows a sequence alignment with (i) the ORF that had the highest BLAST score, ybr293w from  Saccharomyces cerevisiae, which has been classified in cluster II of the subgroup by computer analysis of the budding yeast genome ( 16), and (ii) the tcrC gene product of  Streptomyces aureofaciens, which has been shown to be required for tetracycline resistance ( 7).	gene_phenotype
69287	1	333406	7	NULL	NULL	NULL	NULL	H9438 protein	GP		is similar to					DLD	GP	yeast			NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_295_4_910_s_144	12127981	The H9438 and M2267 proteins share, on average, 28% identity and 48% similarity to three yeast proteins (DLD, AIP2, and YEL071W) that are known to exhibit  -lactate dehydrogenase activity [ 6.	gene_phenotype
69288	2	333406	7	NULL	NULL	NULL	NULL	H9438 protein	GP		is similar to					AIP2	GP	yeast			NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_295_4_910_s_144	12127981	The H9438 and M2267 proteins share, on average, 28% identity and 48% similarity to three yeast proteins (DLD, AIP2, and YEL071W) that are known to exhibit  -lactate dehydrogenase activity [ 6.	gene_phenotype
69289	3	333406	7	NULL	NULL	NULL	NULL	H9438 protein	GP		is similar to					YEL071W	GP	yeast			NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_295_4_910_s_144	12127981	The H9438 and M2267 proteins share, on average, 28% identity and 48% similarity to three yeast proteins (DLD, AIP2, and YEL071W) that are known to exhibit  -lactate dehydrogenase activity [ 6.	gene_phenotype
69290	4	333406	7	NULL	NULL	0	NULL	M2267 protein	GP		is similar to					DLD	GP	yeast			NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_295_4_910_s_144	12127981	The H9438 and M2267 proteins share, on average, 28% identity and 48% similarity to three yeast proteins (DLD, AIP2, and YEL071W) that are known to exhibit  -lactate dehydrogenase activity [ 6.	gene_phenotype
69291	5	333406	7	NULL	NULL	0	NULL	M2267 protein	GP		is similar to					AIP2	GP	yeast			NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_295_4_910_s_144	12127981	The H9438 and M2267 proteins share, on average, 28% identity and 48% similarity to three yeast proteins (DLD, AIP2, and YEL071W) that are known to exhibit  -lactate dehydrogenase activity [ 6.	gene_phenotype
69292	6	333406	7	NULL	NULL	NULL	NULL	M2267 protein	GP		is similar to					YEL071W	GP	yeast			NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_295_4_910_s_144	12127981	The H9438 and M2267 proteins share, on average, 28% identity and 48% similarity to three yeast proteins (DLD, AIP2, and YEL071W) that are known to exhibit  -lactate dehydrogenase activity [ 6.	gene_phenotype
69293	7	333406	7	NULL	NULL	0	NULL	DLD	GP	yeast	activates					lactate dehydrogenase 	GP				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_295_4_910_s_144	12127981	The H9438 and M2267 proteins share, on average, 28% identity and 48% similarity to three yeast proteins (DLD, AIP2, and YEL071W) that are known to exhibit  -lactate dehydrogenase activity [ 6.	gene_phenotype
69294	8	333406	7	NULL	NULL	0	NULL	AIP2	GP	yeast	activates					lactate dehydrogenase 	GP				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_295_4_910_s_144	12127981	The H9438 and M2267 proteins share, on average, 28% identity and 48% similarity to three yeast proteins (DLD, AIP2, and YEL071W) that are known to exhibit  -lactate dehydrogenase activity [ 6.	gene_phenotype
69295	9	333406	7	NULL	NULL	0	NULL	YEL071W	GP	yeast	activates					lactate dehydrogenase 	GP				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_295_4_910_s_144	12127981	The H9438 and M2267 proteins share, on average, 28% identity and 48% similarity to three yeast proteins (DLD, AIP2, and YEL071W) that are known to exhibit  -lactate dehydrogenase activity [ 6.	gene_phenotype
69296	1	333407	7	NULL	NULL	0	NULL	YIL006w	GP		characterized as		functionally			Ndt1p	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_103_8_2617_s_185	16469842	The previously proposed pyruvate carrier, YIL006w, has now been identified and functionally characterized as the mitochondrial NAD carrier protein (Ndt1p) by using transport assays with purified protein reconstituted into liposomes ( ).	gene_phenotype
69297	2	333407	7	NULL	NULL	0	NULL	Ndt1p	GP		is					mitochondrial NAD carrier protein	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_103_8_2617_s_185	16469842	The previously proposed pyruvate carrier, YIL006w, has now been identified and functionally characterized as the mitochondrial NAD carrier protein (Ndt1p) by using transport assays with purified protein reconstituted into liposomes ( ).	gene_phenotype
69298	1	333409	7	NULL	NULL	0	NULL	 Yil007c	GP		interacts with					Chs4	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_154_3_549_s_255	11489916	When used as bait in two-hybrid screens, Yil007c interacted with Chs4 and with Pfs1, a protein required for sporulation ( Deng and Saunders, 2001).	gene_phenotype
69299	2	333409	7	NULL	NULL	0	NULL	Yil007c	GP		interacts with					Pfs1	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_154_3_549_s_255	11489916	When used as bait in two-hybrid screens, Yil007c interacted with Chs4 and with Pfs1, a protein required for sporulation ( Deng and Saunders, 2001).	gene_phenotype
69300	3	333409	7	NULL	NULL	0	NULL	Pfs1 protein	GP		is required for					sporulation	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_154_3_549_s_255	11489916	When used as bait in two-hybrid screens, Yil007c interacted with Chs4 and with Pfs1, a protein required for sporulation ( Deng and Saunders, 2001).	gene_phenotype
69301	1	333410	7	NULL	NULL	0	NULL	Rho1	GP		interacts with					Yil007c	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_154_3_549_s_254	11489916	Rho1 also interacted with a novel protein, Yil007c, which may have a function in regulating cell wall synthesis and other processes during sporulation.	gene_phenotype
69302	2	333410	7	NULL	NULL	NULL	NULL	Yil007c	GP		function in		may			cell wall synthesis	Process	regulating			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_3_549_s_254	11489916	Rho1 also interacted with a novel protein, Yil007c, which may have a function in regulating cell wall synthesis and other processes during sporulation.	gene_phenotype
69303	3	333410	7	NULL	NULL	NULL	NULL	Yil007c	GP		function in		may			sporulation	Process	processes during			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_3_549_s_254	11489916	Rho1 also interacted with a novel protein, Yil007c, which may have a function in regulating cell wall synthesis and other processes during sporulation.	gene_phenotype
69304	4	333410	7	NULL	NULL	0	NULL	Yil007c	GP		is a type of					novel protein	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_154_3_549_s_254	11489916	Rho1 also interacted with a novel protein, Yil007c, which may have a function in regulating cell wall synthesis and other processes during sporulation.	gene_phenotype
69375	1	333412	7	NULL	NULL	NULL	NULL	 Pol32	GP	S. cerevisiae	interacts with					pol alpha	GP		catalytic subunits of		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_8_6285_s_292	15590683	S. cerevisiae protein YJR043C (Pol32) interacts with the catalytic subunits of pol alpha and it is required for the cell cycle progression in G2/M phase ( ).	gene_phenotype
69376	2	333412	7	NULL	NULL	0	NULL	statement 1	Process		is required for					cell cycle	Process	 progression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_8_6285_s_292	15590683	S. cerevisiae protein YJR043C (Pol32) interacts with the catalytic subunits of pol alpha and it is required for the cell cycle progression in G2/M phase ( ).	gene_phenotype
69377	3	333412	7	NULL	NULL	0	NULL	statement 2	Process		occur in					G2/M phase	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_8_6285_s_292	15590683	S. cerevisiae protein YJR043C (Pol32) interacts with the catalytic subunits of pol alpha and it is required for the cell cycle progression in G2/M phase ( ).	gene_phenotype
69378	4	333412	7	NULL	NULL	0	NULL	YJR043C	GP	S. cerevisiae	is					Pol32	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_8_6285_s_292	15590683	S. cerevisiae protein YJR043C (Pol32) interacts with the catalytic subunits of pol alpha and it is required for the cell cycle progression in G2/M phase ( ).	gene_phenotype
69379	1	333414	7	NULL	NULL	0	NULL	Pol32 protein	GP	Saccharomyces cerevisiae	interacts with					DNA polymerase alpha	GP		catalytic subunits of		NULL		0	NULL	NULL	NULL	abs-batch0680-0699_mol-gen-genet_260_6_9928933_s_1	9928933	The Saccharomyces cerevisiae protein YJR043C (Pol32) interacts with the catalytic subunit of DNA polymerase alpha and is required for cell cycle progression in G2/M..	gene_phenotype
69380	2	333414	7	NULL	NULL	0	NULL	statement 1	Process		is required for					cell cycle	Process	progression of			NULL		0	NULL	NULL	NULL	abs-batch0680-0699_mol-gen-genet_260_6_9928933_s_1	9928933	The Saccharomyces cerevisiae protein YJR043C (Pol32) interacts with the catalytic subunit of DNA polymerase alpha and is required for cell cycle progression in G2/M..	gene_phenotype
69381	3	333414	7	NULL	NULL	0	NULL	statement 2	Process		occur in					G2/M 	Process				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_mol-gen-genet_260_6_9928933_s_1	9928933	The Saccharomyces cerevisiae protein YJR043C (Pol32) interacts with the catalytic subunit of DNA polymerase alpha and is required for cell cycle progression in G2/M..	gene_phenotype
69382	4	333414	7	NULL	NULL	0	NULL	Pol32	GP		is					YJR043C	GP				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_mol-gen-genet_260_6_9928933_s_1	9928933	The Saccharomyces cerevisiae protein YJR043C (Pol32) interacts with the catalytic subunit of DNA polymerase alpha and is required for cell cycle progression in G2/M..	gene_phenotype
69383	1	333415	7	NULL	NULL	0	NULL	YJR043c ORF 	GP	sequence upstream of	reveals								MluI motif (ACGCGT)		NULL		0	NULL	NULL	NULL	abs-batch0680-0699_mol-gen-genet_260_6_9928933_s_10	9928933	Analysis  of the sequence upstream of the YJR043c ORF revealed the presence of an  MluI motif (ACGCGT), a sequence associated with many genes involved in  DNA replication in budding yeast.	gene_phenotype
69384	2	333415	7	NULL	NULL	0	NULL				associate with			MluI motif (ACGCGT)		DNA replication genes	GP	budding yeast			NULL		0	NULL	NULL	NULL	abs-batch0680-0699_mol-gen-genet_260_6_9928933_s_10	9928933	Analysis  of the sequence upstream of the YJR043c ORF revealed the presence of an  MluI motif (ACGCGT), a sequence associated with many genes involved in  DNA replication in budding yeast.	gene_phenotype
69385	1	333417	7	NULL	NULL	0	NULL	MPT5	GP		is a type of					RNA-binding proteins	GP		Puf family		NULL		0	NULL	NULL	NULL	gw60_embo_20_3_552_s_42	11157761	We examined  HO expression and  ASH1 mRNA localization in yeast mutants lacking each of the five genes coding for members of the Puf family of RNA-binding proteins:  MPT5,  YGL014w,  YLL013c,  JSN1 and  YPR039c.	gene_phenotype
69386	2	333417	7	NULL	NULL	0	NULL	YGL014w	GP		is a type of					RNA-binding proteins	GP		Puf family		NULL		0	NULL	NULL	NULL	gw60_embo_20_3_552_s_42	11157761	We examined  HO expression and  ASH1 mRNA localization in yeast mutants lacking each of the five genes coding for members of the Puf family of RNA-binding proteins:  MPT5,  YGL014w,  YLL013c,  JSN1 and  YPR039c.	gene_phenotype
69387	3	333417	7	NULL	NULL	0	NULL	YLL013c	GP		is a type of					RNA-binding proteins	GP		Puf family		NULL		0	NULL	NULL	NULL	gw60_embo_20_3_552_s_42	11157761	We examined  HO expression and  ASH1 mRNA localization in yeast mutants lacking each of the five genes coding for members of the Puf family of RNA-binding proteins:  MPT5,  YGL014w,  YLL013c,  JSN1 and  YPR039c.	gene_phenotype
69388	4	333417	7	NULL	NULL	0	NULL	JSN1	GP		is a type of					RNA-binding proteins	GP		Puf family		NULL		0	NULL	NULL	NULL	gw60_embo_20_3_552_s_42	11157761	We examined  HO expression and  ASH1 mRNA localization in yeast mutants lacking each of the five genes coding for members of the Puf family of RNA-binding proteins:  MPT5,  YGL014w,  YLL013c,  JSN1 and  YPR039c.	gene_phenotype
69389	5	333417	7	NULL	NULL	0	NULL	YPR039c	GP		is a type of					RNA-binding proteins	GP		Puf family		NULL		0	NULL	NULL	NULL	gw60_embo_20_3_552_s_42	11157761	We examined  HO expression and  ASH1 mRNA localization in yeast mutants lacking each of the five genes coding for members of the Puf family of RNA-binding proteins:  MPT5,  YGL014w,  YLL013c,  JSN1 and  YPR039c.	gene_phenotype
69390	1	333418	7	NULL	NULL	0	NULL	protein	GP		transported from					endoplasmic reticulum	CellComponent				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_10_6796_s_151	10490618	During the course of our study, Chen and coworkers ( 8) independently identified scSAP 130 as a protein, RSE1 (YML049c), in a screen of temperature-sensitive mutants defective in endoplasmic reticulum-to-golgi transport.	gene_phenotype
69391	2	333418	7	NULL	NULL	0	NULL	Protein	GP		transported to					golgi 	CellComponent				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_10_6796_s_151	10490618	During the course of our study, Chen and coworkers ( 8) independently identified scSAP 130 as a protein, RSE1 (YML049c), in a screen of temperature-sensitive mutants defective in endoplasmic reticulum-to-golgi transport.	gene_phenotype
69392	3	333418	7	NULL	NULL	0	NULL	statement 1			occur along with					statement 2					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_10_6796_s_151	10490618	During the course of our study, Chen and coworkers ( 8) independently identified scSAP 130 as a protein, RSE1 (YML049c), in a screen of temperature-sensitive mutants defective in endoplasmic reticulum-to-golgi transport.	gene_phenotype
69393	4	333418	7	NULL	NULL	0	NULL	scSAP130	GP		defective in					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_10_6796_s_151	10490618	During the course of our study, Chen and coworkers ( 8) independently identified scSAP 130 as a protein, RSE1 (YML049c), in a screen of temperature-sensitive mutants defective in endoplasmic reticulum-to-golgi transport.	gene_phenotype
69394	2	333419	7	NULL	NULL	NULL	NULL	ESA1	GP		is essential for					 cellular viability	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_4_2515_s_97	10082517	Thus, the YOR244w gene product is essential for cellular viability, and we have named it  ESA1, for essential  SAS family acetyltransferase.	gene_phenotype
69395	1	333419	7	NULL	NULL	0	NULL	YOR244w gene product	GP		is					ESA1	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_4_2515_s_97	10082517	Thus, the YOR244w gene product is essential for cellular viability, and we have named it  ESA1, for essential  SAS family acetyltransferase.	gene_phenotype
69396	3	333419	7	NULL	NULL	0	NULL	ESA1	GP		is					essential SAS family acetyltransferase	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_4_2515_s_97	10082517	Thus, the YOR244w gene product is essential for cellular viability, and we have named it  ESA1, for essential  SAS family acetyltransferase.	gene_phenotype
69397	1	333420	7	NULL	NULL	0	NULL	YOR244w ORF	GP		existed on					chromosome XV	Chromosome	yeast			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_4_2515_s_90	10082517	During analysis of the yeast  SAS2 and  SAS3 silencing genes ( 53), we discovered that another, very similar but previously uncharacterized open reading frame (ORF) (YOR244w) existed on yeast chromosome XV.	gene_phenotype
69398	2	333420	7	NULL	NULL	0	NULL	ORF	GP		is 					open reading frame	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_4_2515_s_90	10082517	During analysis of the yeast  SAS2 and  SAS3 silencing genes ( 53), we discovered that another, very similar but previously uncharacterized open reading frame (ORF) (YOR244w) existed on yeast chromosome XV.	gene_phenotype
69399	1	333421	7	NULL	NULL	0	NULL	YDR409W	GP	budding yeast	belongs to					PIAS family	GP				NULL		0	NULL	NULL	NULL	gw60_molcell_8_3_713_s_91	11583632	YDR409W of budding yeast,  Saccharomyces cerevisiae, also belongs to this PIAS family.	gene_phenotype
69400	2	333421	7	NULL	NULL	0	NULL	YDR409W	GP	Saccharomyces cerevisiae	belongs to					PIAS family	GP				NULL		0	NULL	NULL	NULL	gw60_molcell_8_3_713_s_91	11583632	YDR409W of budding yeast,  Saccharomyces cerevisiae, also belongs to this PIAS family.	gene_phenotype
69401	1	333422	7	NULL	NULL	0	NULL	YDR409w	GP	budding yeast	is					Siz1/Ull1	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_52_48973_s_4	11577116	In our previous report (Takahashi, Y., Toh-e, A., and Kikuchi, Y. (2001)  Gene 275, 223-231), we showed that Siz1/Ull1 (YDR409w) of budding yeast, a member of the human PIAS family containing a RING-like domain, is a strong candidate for SUMO1/Smt3 ligase because the SUMO1/Smt3 modification of septin components was abolished in the  ull1 mutant and Ull1 associated with E2 (Ubc9) and the substrates (septin components) in immunoprecipitation experiments.	gene_phenotype
69402	2	333422	7	NULL	NULL	0	NULL	Siz1/Ull1	GP		is a member of					PIAS family 	GP	human			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_52_48973_s_4	11577116	In our previous report (Takahashi, Y., Toh-e, A., and Kikuchi, Y. (2001)  Gene 275, 223-231), we showed that Siz1/Ull1 (YDR409w) of budding yeast, a member of the human PIAS family containing a RING-like domain, is a strong candidate for SUMO1/Smt3 ligase because the SUMO1/Smt3 modification of septin components was abolished in the  ull1 mutant and Ull1 associated with E2 (Ubc9) and the substrates (septin components) in immunoprecipitation experiments.	gene_phenotype
69403	3	333422	7	NULL	NULL	0	NULL	PIAS family 	GP	human	contain					RING-like domain	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_52_48973_s_4	11577116	In our previous report (Takahashi, Y., Toh-e, A., and Kikuchi, Y. (2001)  Gene 275, 223-231), we showed that Siz1/Ull1 (YDR409w) of budding yeast, a member of the human PIAS family containing a RING-like domain, is a strong candidate for SUMO1/Smt3 ligase because the SUMO1/Smt3 modification of septin components was abolished in the  ull1 mutant and Ull1 associated with E2 (Ubc9) and the substrates (septin components) in immunoprecipitation experiments.	gene_phenotype
69404	4	333422	7	NULL	NULL	0	NULL	Siz1/Ull1	GP		is a candidate for		strong			SUMO1/Smt3 ligase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_52_48973_s_4	11577116	In our previous report (Takahashi, Y., Toh-e, A., and Kikuchi, Y. (2001)  Gene 275, 223-231), we showed that Siz1/Ull1 (YDR409w) of budding yeast, a member of the human PIAS family containing a RING-like domain, is a strong candidate for SUMO1/Smt3 ligase because the SUMO1/Smt3 modification of septin components was abolished in the  ull1 mutant and Ull1 associated with E2 (Ubc9) and the substrates (septin components) in immunoprecipitation experiments.	gene_phenotype
69405	5	333422	7	NULL	NULL	NULL	NULL	SUMO1/Smt3	GP	modification of 	is abolished in			septin components of		ull1	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_52_48973_s_4	11577116	In our previous report (Takahashi, Y., Toh-e, A., and Kikuchi, Y. (2001)  Gene 275, 223-231), we showed that Siz1/Ull1 (YDR409w) of budding yeast, a member of the human PIAS family containing a RING-like domain, is a strong candidate for SUMO1/Smt3 ligase because the SUMO1/Smt3 modification of septin components was abolished in the  ull1 mutant and Ull1 associated with E2 (Ubc9) and the substrates (septin components) in immunoprecipitation experiments.	gene_phenotype
69406	6	333422	7	NULL	NULL	0	NULL	Ull1 	GP		associate with					E2	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_52_48973_s_4	11577116	In our previous report (Takahashi, Y., Toh-e, A., and Kikuchi, Y. (2001)  Gene 275, 223-231), we showed that Siz1/Ull1 (YDR409w) of budding yeast, a member of the human PIAS family containing a RING-like domain, is a strong candidate for SUMO1/Smt3 ligase because the SUMO1/Smt3 modification of septin components was abolished in the  ull1 mutant and Ull1 associated with E2 (Ubc9) and the substrates (septin components) in immunoprecipitation experiments.	gene_phenotype
69407	7	333422	7	NULL	NULL	0	NULL	E2	GP		is					Ubc9	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_52_48973_s_4	11577116	In our previous report (Takahashi, Y., Toh-e, A., and Kikuchi, Y. (2001)  Gene 275, 223-231), we showed that Siz1/Ull1 (YDR409w) of budding yeast, a member of the human PIAS family containing a RING-like domain, is a strong candidate for SUMO1/Smt3 ligase because the SUMO1/Smt3 modification of septin components was abolished in the  ull1 mutant and Ull1 associated with E2 (Ubc9) and the substrates (septin components) in immunoprecipitation experiments.	gene_phenotype
69408	8	333422	7	NULL	NULL	0	NULL	Ull1 	GP		associate with					septin components	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_52_48973_s_4	11577116	In our previous report (Takahashi, Y., Toh-e, A., and Kikuchi, Y. (2001)  Gene 275, 223-231), we showed that Siz1/Ull1 (YDR409w) of budding yeast, a member of the human PIAS family containing a RING-like domain, is a strong candidate for SUMO1/Smt3 ligase because the SUMO1/Smt3 modification of septin components was abolished in the  ull1 mutant and Ull1 associated with E2 (Ubc9) and the substrates (septin components) in immunoprecipitation experiments.	gene_phenotype
69409	1	333423	7	NULL	NULL	0	NULL	PEA2 YER149c	GP		localized with					Spa2p	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_211	15334557	PEA2   YER149c Localized with Spa2p to sites of polarized growth and required for efficient mating,  bipolar budding and pheromone-induced shmoo formation	gene_phenotype
69410	2	333423	7	NULL	NULL	NULL	NULL	statement 1	Process		localized to					polarized growth	Process	sites of			NULL		NULL	NULL	NULL	NULL	gw70_yeast_21_11_927_s_211	15334557	PEA2   YER149c Localized with Spa2p to sites of polarized growth and required for efficient mating,  bipolar budding and pheromone-induced shmoo formation	gene_phenotype
69411	3	333423	7	NULL	NULL	0	NULL	statement 2	Process		required for					mating	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_211	15334557	PEA2   YER149c Localized with Spa2p to sites of polarized growth and required for efficient mating,  bipolar budding and pheromone-induced shmoo formation	gene_phenotype
69412	4	333423	7	NULL	NULL	NULL	NULL	statement 2	Process		required for					bipolar budding	Process				NULL		NULL	NULL	NULL	NULL	gw70_yeast_21_11_927_s_211	15334557	PEA2   YER149c Localized with Spa2p to sites of polarized growth and required for efficient mating,  bipolar budding and pheromone-induced shmoo formation	gene_phenotype
69413	5	333423	7	NULL	NULL	0	NULL	pheromone	GP		induce					shmoo formation	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_211	15334557	PEA2   YER149c Localized with Spa2p to sites of polarized growth and required for efficient mating,  bipolar budding and pheromone-induced shmoo formation	gene_phenotype
69414	6	333423	7	NULL	NULL	0	NULL	statement 2	Process		required for					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_211	15334557	PEA2   YER149c Localized with Spa2p to sites of polarized growth and required for efficient mating,  bipolar budding and pheromone-induced shmoo formation	gene_phenotype
69415	1	333424	7	NULL	NULL	0	NULL	PEA2 YER149C	GP		involved in					orientated growth	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_154	15645503	PEA2  YER149C Involved in orientated growth toward mating partner, required for stimulation of the  low-affinity Ca2+ in flux system that is activated in response to mating pheromone and is required  for cell-cell fusion (Sheu  et al., [ 2000])	gene_phenotype
69416	2	333424	7	NULL	NULL	0	NULL	statement 1	Process		toward					mating partner	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_154	15645503	PEA2  YER149C Involved in orientated growth toward mating partner, required for stimulation of the  low-affinity Ca2+ in flux system that is activated in response to mating pheromone and is required  for cell-cell fusion (Sheu  et al., [ 2000])	gene_phenotype
69417	3	333424	7	NULL	NULL	NULL	NULL	PEA2 YER149C	GP		required for					Ca2+ influx system	Process	stimulation of low-affinity			NULL		NULL	NULL	NULL	NULL	gw70_yeast_22_2_79_s_154	15645503	PEA2  YER149C Involved in orientated growth toward mating partner, required for stimulation of the  low-affinity Ca2+ in flux system that is activated in response to mating pheromone and is required  for cell-cell fusion (Sheu  et al., [ 2000])	gene_phenotype
69418	4	333424	7	NULL	NULL	0	NULL	 Ca2+ in flux system	Process		activated in					mating pheromone	GP	response to			NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_154	15645503	PEA2  YER149C Involved in orientated growth toward mating partner, required for stimulation of the  low-affinity Ca2+ in flux system that is activated in response to mating pheromone and is required  for cell-cell fusion (Sheu  et al., [ 2000])	gene_phenotype
69419	5	333424	7	NULL	NULL	0	NULL	 Ca2+ in flux system	Process		required for					cell-cell fusion	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_154	15645503	PEA2  YER149C Involved in orientated growth toward mating partner, required for stimulation of the  low-affinity Ca2+ in flux system that is activated in response to mating pheromone and is required  for cell-cell fusion (Sheu  et al., [ 2000])	gene_phenotype
69678	1	333426	6	NULL	NULL	0	NULL	YHL007c STE20	GP		is involved in					pheromone response	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_73	16498703	YHL007c   STE20 Signal transducing kinase of the PAK (p21-activated kinase) family, involved in pheromone  response and pseudohyphal/invasive growth pathways, activated by Cdc42p; binds Ste4p  at a GBB motif present in non-catalytic domains of PAK kinases  [ 44]	gene_phenotype
69679	2	333426	6	NULL	NULL	0	NULL	YHL007c STE20	GP		is a type of					PAK 	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_73	16498703	YHL007c   STE20 Signal transducing kinase of the PAK (p21-activated kinase) family, involved in pheromone  response and pseudohyphal/invasive growth pathways, activated by Cdc42p; binds Ste4p  at a GBB motif present in non-catalytic domains of PAK kinases  [ 44]	gene_phenotype
69680	3	333426	6	NULL	NULL	0	NULL	PAK	GP		is					p21-activated kinase	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_73	16498703	YHL007c   STE20 Signal transducing kinase of the PAK (p21-activated kinase) family, involved in pheromone  response and pseudohyphal/invasive growth pathways, activated by Cdc42p; binds Ste4p  at a GBB motif present in non-catalytic domains of PAK kinases  [ 44]	gene_phenotype
69681	4	333426	6	NULL	NULL	0	NULL	YHL007c STE20	GP		is involved in					pseudohyphal/invasive growth pathways	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_73	16498703	YHL007c   STE20 Signal transducing kinase of the PAK (p21-activated kinase) family, involved in pheromone  response and pseudohyphal/invasive growth pathways, activated by Cdc42p; binds Ste4p  at a GBB motif present in non-catalytic domains of PAK kinases  [ 44]	gene_phenotype
69682	5	333426	6	NULL	NULL	0	NULL	YHL007c STE20	GP		bind					Ste4p	GP			GBB motif	NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_73	16498703	YHL007c   STE20 Signal transducing kinase of the PAK (p21-activated kinase) family, involved in pheromone  response and pseudohyphal/invasive growth pathways, activated by Cdc42p; binds Ste4p  at a GBB motif present in non-catalytic domains of PAK kinases  [ 44]	gene_phenotype
69683	6	333426	6	NULL	NULL	NULL	NULL	YHL007c STE20	GP		is activated by					Cdc42p	GP				NULL		NULL	NULL	NULL	NULL	gw70_yeast_23_3_159_s_73	16498703	YHL007c   STE20 Signal transducing kinase of the PAK (p21-activated kinase) family, involved in pheromone  response and pseudohyphal/invasive growth pathways, activated by Cdc42p; binds Ste4p  at a GBB motif present in non-catalytic domains of PAK kinases  [ 44]	gene_phenotype
69684	7	333426	6	NULL	NULL	0	NULL	GBB motif 			is present in					PAK kinase	GP		non-catalytic domain		NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_73	16498703	YHL007c   STE20 Signal transducing kinase of the PAK (p21-activated kinase) family, involved in pheromone  response and pseudohyphal/invasive growth pathways, activated by Cdc42p; binds Ste4p  at a GBB motif present in non-catalytic domains of PAK kinases  [ 44]	gene_phenotype
69685	1	333428	6	NULL	NULL	NULL	NULL	Yil159w Bnr1 1 Formin	GP		nucleates					linear actin filaments	CellComponent	formation of 			NULL		NULL	NULL	NULL	NULL	gw70_yeast_23_3_159_s_140	16498703	Yil159w  Bnr1  1 Formin, nucleates the formation of linear actin filaments, involved in cell processes  such as budding and mitotic spindle orientation, which require the formation of polarized  actin cables; functionally redundant with  BNI1  LIP  [ 20]	gene_phenotype
69686	2	333428	6	NULL	NULL	0	NULL	Yil159w Bnr1 1 Formin	GP		is involved in					budding	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_140	16498703	Yil159w  Bnr1  1 Formin, nucleates the formation of linear actin filaments, involved in cell processes  such as budding and mitotic spindle orientation, which require the formation of polarized  actin cables; functionally redundant with  BNI1  LIP  [ 20]	gene_phenotype
69687	3	333428	6	NULL	NULL	0	NULL	Yil159w Bnr1 1 Formin	GP		is involved in					mitotic spindle	CellComponent	orientation of			NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_140	16498703	Yil159w  Bnr1  1 Formin, nucleates the formation of linear actin filaments, involved in cell processes  such as budding and mitotic spindle orientation, which require the formation of polarized  actin cables; functionally redundant with  BNI1  LIP  [ 20]	gene_phenotype
69688	4	333428	6	NULL	NULL	0	NULL	linear actin filaments	CellComponent		ia required for					actin cables	CellComponent	formation of;; polarized			NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_140	16498703	Yil159w  Bnr1  1 Formin, nucleates the formation of linear actin filaments, involved in cell processes  such as budding and mitotic spindle orientation, which require the formation of polarized  actin cables; functionally redundant with  BNI1  LIP  [ 20]	gene_phenotype
69689	5	333428	6	NULL	NULL	0	NULL	Yil159w Bnr1 1 Formin	GP		is functionally redundant with					BNI1 LIP	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_140	16498703	Yil159w  Bnr1  1 Formin, nucleates the formation of linear actin filaments, involved in cell processes  such as budding and mitotic spindle orientation, which require the formation of polarized  actin cables; functionally redundant with  BNI1  LIP  [ 20]	gene_phenotype
69690	1	333429	6	NULL	NULL	0	NULL	YJL094c	GP		shows closest homology to					KefC	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_12_6951_s_232	9507001	Of these, YJL094c also shows closest homology to a glutathione-regulated K+ efflux transporter (KefC) from  Escherichia coli ( 65), although it does not appear to contain a putative mitochondrial targeting signal at its N terminus.	gene_phenotype
69691	2	333429	6	NULL	NULL	NULL	NULL	KefC	GP		is					K+ efflux transporter	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_12_6951_s_232	9507001	Of these, YJL094c also shows closest homology to a glutathione-regulated K+ efflux transporter (KefC) from  Escherichia coli ( 65), although it does not appear to contain a putative mitochondrial targeting signal at its N terminus.	gene_phenotype
69704	3	333429	6	NULL	NULL	0	NULL	YJL094c	GP		does not contain					mitochondrial targeting signal	AminoAcid	putative	N terminus		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_12_6951_s_232	9507001	Of these, YJL094c also shows closest homology to a glutathione-regulated K+ efflux transporter (KefC) from  Escherichia coli ( 65), although it does not appear to contain a putative mitochondrial targeting signal at its N terminus.	gene_phenotype
69706	1	333430	6	NULL	NULL	0	NULL	YKR081c	GP		is necessary for					vegetative cell growth	Process				NULL		0	NULL	NULL	NULL	gw60_gene_233_1_141_s_152	10375630	This fact undoubtedly confirms that  YKR081c and  YKR083c are necessary for vegetative cell growth.	gene_phenotype
69708	2	333430	6	NULL	NULL	0	NULL	YKR083c	GP		is necessary for					vegetative cell growth	Process				NULL		0	NULL	NULL	NULL	gw60_gene_233_1_141_s_152	10375630	This fact undoubtedly confirms that  YKR081c and  YKR083c are necessary for vegetative cell growth.	gene_phenotype
69709	1	333431	6	NULL	NULL	0	NULL	YKR081c	GP		is necessary for					vegetative growth	Process				NULL		0	NULL	NULL	NULL	gw60_gene_233_1_141_s_124	10375630	Functional analysis of deletion FYBL3/Jz024:  YKR081c and  YKR083c are essential for vegetative growth;  YKR082c deletion renders heat-sensitive mutants	gene_phenotype
69712	2	333431	6	NULL	NULL	0	NULL	YKR083c	GP		is necessary for					vegetative growth	Process				NULL		0	NULL	NULL	NULL	gw60_gene_233_1_141_s_124	10375630	Functional analysis of deletion FYBL3/Jz024:  YKR081c and  YKR083c are essential for vegetative growth;  YKR082c deletion renders heat-sensitive mutants	gene_phenotype
69713	3	333431	6	NULL	NULL	0	NULL	YKR082c	GP	deletion of	renders					heat-sensitive mutant					NULL		0	NULL	NULL	NULL	gw60_gene_233_1_141_s_124	10375630	Functional analysis of deletion FYBL3/Jz024:  YKR081c and  YKR083c are essential for vegetative growth;  YKR082c deletion renders heat-sensitive mutants	gene_phenotype
69715	1	333432	6	NULL	NULL	NULL	NULL	bilirubin	GP	Saccharomyces cerevisiae;; unconjugated	is transported to					vacuoles	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_16_4761_s_481	11466279	The products of YCF1 and YLL015w (BPT1) cooperate for the ATP-dependent vacuolar transport of unconjugated bilirubin in  Saccharomyces cerevisiae.	gene_phenotype
69718	2	333432	6	NULL	NULL	0	NULL	YCF1 product	GP		cooperates for					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_16_4761_s_481	11466279	The products of YCF1 and YLL015w (BPT1) cooperate for the ATP-dependent vacuolar transport of unconjugated bilirubin in  Saccharomyces cerevisiae.	gene_phenotype
69719	3	333432	6	NULL	NULL	0	NULL	YLL015w product	GP		cooperates for					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_16_4761_s_481	11466279	The products of YCF1 and YLL015w (BPT1) cooperate for the ATP-dependent vacuolar transport of unconjugated bilirubin in  Saccharomyces cerevisiae.	gene_phenotype
69720	4	333432	6	NULL	NULL	0	NULL	statement 1	Process		is dependent on					ATP	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_16_4761_s_481	11466279	The products of YCF1 and YLL015w (BPT1) cooperate for the ATP-dependent vacuolar transport of unconjugated bilirubin in  Saccharomyces cerevisiae.	gene_phenotype
69721	1	333433	6	NULL	NULL	0	NULL	Bpt1p	GP		localizes to					vacuoles	CellComponent				NULL		0	NULL	NULL	NULL	gw60_febslett_520_1_63_s_68	12044871	A previous study characterized Bpt1p ( YLL015w) as a transporter mediating uptake of unconjugated bilirubins into vacuolar vesicles [ 30], implying vacuolar localization of Bpt1p.	gene_phenotype
69722	2	333433	6	NULL	NULL	0	NULL	bilirubins	GP	unconjugated	are tranported to					vacuolar vesicles	CellComponent				NULL		0	NULL	NULL	NULL	gw60_febslett_520_1_63_s_68	12044871	A previous study characterized Bpt1p ( YLL015w) as a transporter mediating uptake of unconjugated bilirubins into vacuolar vesicles [ 30], implying vacuolar localization of Bpt1p.	gene_phenotype
69724	3	333433	6	NULL	NULL	NULL	NULL	Bpt1p ( YLL015w)	GP		mediates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_520_1_63_s_68	12044871	A previous study characterized Bpt1p ( YLL015w) as a transporter mediating uptake of unconjugated bilirubins into vacuolar vesicles [ 30], implying vacuolar localization of Bpt1p.	gene_phenotype
69732	1	333435	6	NULL	NULL	0	NULL	Bpt1p	GP		is					bile pigment transporter-1	GP				NULL		0	NULL	NULL	NULL	gw60_febslett_520_1_63_s_21	12044871	Furthermore, Bpt1p (bile pigment transporter-1/ YLL015w), the closest yeast homologue of Ycf1p, was originally discovered as a pump mediating vacuolar uptake of unconjugated bile pigments and magnetic resonance contrast agents [  30 and   31].	gene_phenotype
69733	2	333435	6	NULL	NULL	0	NULL	Bpt1p	GP		is homologue of 					Ycf1	GP				NULL		0	NULL	NULL	NULL	gw60_febslett_520_1_63_s_21	12044871	Furthermore, Bpt1p (bile pigment transporter-1/ YLL015w), the closest yeast homologue of Ycf1p, was originally discovered as a pump mediating vacuolar uptake of unconjugated bile pigments and magnetic resonance contrast agents [  30 and   31].	gene_phenotype
69736	3	333435	6	NULL	NULL	0	NULL	vacuoles	CellComponent		uptake					bile pigments	unconjugated				NULL		0	NULL	NULL	NULL	gw60_febslett_520_1_63_s_21	12044871	Furthermore, Bpt1p (bile pigment transporter-1/ YLL015w), the closest yeast homologue of Ycf1p, was originally discovered as a pump mediating vacuolar uptake of unconjugated bile pigments and magnetic resonance contrast agents [  30 and   31].	gene_phenotype
69738	4	333435	6	NULL	NULL	0	NULL	Bpt1p	GP		mediates					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_520_1_63_s_21	12044871	Furthermore, Bpt1p (bile pigment transporter-1/ YLL015w), the closest yeast homologue of Ycf1p, was originally discovered as a pump mediating vacuolar uptake of unconjugated bile pigments and magnetic resonance contrast agents [  30 and   31].	gene_phenotype
69743	1	333437	6	NULL	NULL	0	NULL	LIF1 		transcriptional repression of	causes					NHEJ 		regulation of;; mating-type-dependent			NULL		0	NULL	NULL	NULL	gw60_nature_414_6864_666_s_14	11740566	Here we report that mating-type-dependent regulation of NHEJ in budding yeast is caused in part by transcriptional repression of both  LIF1 and the gene  NEJ1 (YLR265C) -- identified from microarray screening of messenger RNAs.	gene_phenotype
69746	2	333437	6	NULL	NULL	0	NULL	NEJ1 (YLR265C)	GP		causes					NHEJ	GP	regulation of;; mating-type-dependent			NULL		0	NULL	NULL	NULL	gw60_nature_414_6864_666_s_14	11740566	Here we report that mating-type-dependent regulation of NHEJ in budding yeast is caused in part by transcriptional repression of both  LIF1 and the gene  NEJ1 (YLR265C) -- identified from microarray screening of messenger RNAs.	gene_phenotype
69783	1	333439	6	NULL	NULL	0	NULL	neural crest cell	Cell		are present 					otic vesicle	CellComponent	anterior to			NULL		0	NULL	NULL	NULL	gw60_genesdev_17_1_141_s_124	12514106	Interestingly, more neural crest cells were observed anterior to the otic vesicle in a region next to the second branchial arch in the  Fgfr1n7/n7 mutants compared with the wild-type embryos.	gene_phenotype
69784	2	333439	6	NULL	NULL	0	NULL	otic vesicle	OrganismPart		is present 					second branchial arch	OrganismPart				NULL	Fgfr1n7/n7 mutants 	0	NULL	NULL	NULL	gw60_genesdev_17_1_141_s_124	12514106	Interestingly, more neural crest cells were observed anterior to the otic vesicle in a region next to the second branchial arch in the  Fgfr1n7/n7 mutants compared with the wild-type embryos.	gene_phenotype
69785	1	333440	6	NULL	NULL	0	NULL	cdc15p			is involved in					cytokinesis					NULL	Schizosaccharomyces pombe	0	NULL	NULL	NULL	gw60_jbiolchem_273_43_28341_s_73	9774458	Ymr032wp is homologous to cdc15p, which is involved in cytokinesis in  Schizosaccharomyces pombe ( 29).	gene_phenotype
69786	2	333440	6	NULL	NULL	0	NULL	Ymr032wp			is homologous to					cdc15p					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_43_28341_s_73	9774458	Ymr032wp is homologous to cdc15p, which is involved in cytokinesis in  Schizosaccharomyces pombe ( 29).	gene_phenotype
69787	1	333441	6	NULL	NULL	0	NULL	Ymr032wp			is homologous to					cdc15p					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_43_28341_s_7	9774458	Ymr032wp was homologous to cdc15p, which is involved in cytokinesis in  Schizosaccharomyces pombe, and we named this gene  HOF1 (homolog of cdc 15).	gene_phenotype
69788	2	333441	6	NULL	NULL	0	NULL	Ymr032wp			is 					HOF1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_43_28341_s_7	9774458	Ymr032wp was homologous to cdc15p, which is involved in cytokinesis in  Schizosaccharomyces pombe, and we named this gene  HOF1 (homolog of cdc 15).	gene_phenotype
69789	3	333441	6	NULL	NULL	0	NULL	HOF1			is					homolog of cdc 15					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_43_28341_s_7	9774458	Ymr032wp was homologous to cdc15p, which is involved in cytokinesis in  Schizosaccharomyces pombe, and we named this gene  HOF1 (homolog of cdc 15).	gene_phenotype
69790	3	333441	6	NULL	NULL	0	NULL	HOF1			is					homolog of cdc 15					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_43_28341_s_7	9774458	Ymr032wp was homologous to cdc15p, which is involved in cytokinesis in  Schizosaccharomyces pombe, and we named this gene  HOF1 (homolog of cdc 15).	gene_phenotype
69791	4	333441	6	NULL	NULL	0	NULL	cdc15p			is involved in					cytokinesis					NULL	Schizosaccharomyces pombe	0	NULL	NULL	NULL	gw60_jbiolchem_273_43_28341_s_7	9774458	Ymr032wp was homologous to cdc15p, which is involved in cytokinesis in  Schizosaccharomyces pombe, and we named this gene  HOF1 (homolog of cdc 15).	gene_phenotype
69792	1	333444	6	NULL	NULL	0	NULL	Ydl119c	GP		is a member of					mitochondrial carrier family of membrane transporters	GP				NULL		0	NULL	NULL	NULL	gw60_chembiol_10_6_521_s_159	12837385	A strain deleted for Ydl119c, a member of the mitochondrial carrier family of membrane transporters, which are involved in the transport of a number of different metabolites across the inner mitochondrial membrane   [25, 26]  , is sensitive to SFK1.	gene_phenotype
69793	2	333444	6	NULL	NULL	0	NULL	Ydl119c	GP	deletion mutant	is sensitive to					SFK1	Chemical				NULL		0	NULL	NULL	NULL	gw60_chembiol_10_6_521_s_159	12837385	A strain deleted for Ydl119c, a member of the mitochondrial carrier family of membrane transporters, which are involved in the transport of a number of different metabolites across the inner mitochondrial membrane   [25, 26]  , is sensitive to SFK1.	gene_phenotype
69794	3	333444	6	NULL	NULL	0	NULL	metabolites	Chemical		transported across					mitochondrial membrane 	CellComponent	inner 			NULL		0	NULL	NULL	NULL	gw60_chembiol_10_6_521_s_159	12837385	A strain deleted for Ydl119c, a member of the mitochondrial carrier family of membrane transporters, which are involved in the transport of a number of different metabolites across the inner mitochondrial membrane   [25, 26]  , is sensitive to SFK1.	gene_phenotype
69805	1	333445	6	NULL	NULL	NULL	NULL	Ggc1p			clusters together with					transporters for nucleotides					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_20_20850_s_224	14998997	In a phylogenetic tree of the  S. cerevisiae members of the mitochondrial carrier family ( ,  ), Ggc1p clusters together with transporters for nucleotides or nucleotide analogs (the three isoforms of the ADP/ATP carrier (  -  ) and the carriers for coenzyme A ( ) and for thiamine pyrophosphate ( ) and with YDL119c (20% identity), which has not yet been identified).	gene_phenotype
69807	2	333445	6	NULL	NULL	0	NULL	Ggc1p			clusters together with					nucleotide analogs					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_20_20850_s_224	14998997	In a phylogenetic tree of the  S. cerevisiae members of the mitochondrial carrier family ( ,  ), Ggc1p clusters together with transporters for nucleotides or nucleotide analogs (the three isoforms of the ADP/ATP carrier (  -  ) and the carriers for coenzyme A ( ) and for thiamine pyrophosphate ( ) and with YDL119c (20% identity), which has not yet been identified).	gene_phenotype
69812	1	333446	6	NULL	NULL	0	NULL	FOB1	GP	wild type	interacts with					FOB1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_3_1932_s_214	14576157	Two-hybrid analyses of protein-protein interactions between wild type  FOB1 or  YDR026C and  FOB1 or its mutant forms and lack of replication fork arrest activity of  YDR026C.	gene_phenotype
69813	2	333446	6	NULL	NULL	0	NULL	YDR026C 	GP	wild type	bind					FOB1	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_3_1932_s_214	14576157	Two-hybrid analyses of protein-protein interactions between wild type  FOB1 or  YDR026C and  FOB1 or its mutant forms and lack of replication fork arrest activity of  YDR026C.	gene_phenotype
69845	1	333447	6	NULL	NULL	0	NULL	Fob1p	GP	mutant	bind					protein encoded in the locus YDR026C	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_3_1932_s_8	14576157	The mutant did not diminish nucleolar transport, and interaction of the mutant form of Fob1p with itself and with another protein encoded in the locus  YDR026C suggested that the mutation did not cause global misfolding of the protein.	gene_phenotype
69846	1	333448	6	NULL	NULL	0	NULL	Nmd3	GP		is a type of					export adapter					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_10_3718_s_29	16648468	For the large subunit, these include the export adapter Nmd3 that provides the nuclear export signal ( ), Tif6 ( ), the uncharacterized protein Arx1 (encoded by YDR101c) ( ), and Rlp24, related to Rpl24 found in mature subunits ( ).	gene_phenotype
69847	2	333448	6	NULL	NULL	NULL	NULL	Nmd3	GP		provides					nuclear export signal	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_10_3718_s_29	16648468	For the large subunit, these include the export adapter Nmd3 that provides the nuclear export signal ( ), Tif6 ( ), the uncharacterized protein Arx1 (encoded by YDR101c) ( ), and Rlp24, related to Rpl24 found in mature subunits ( ).	gene_phenotype
69848	1	333449	6	NULL	NULL	NULL	NULL	Nmd3	GP		is a type of					nuclear export factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_20_5539_s_180	12374754	The nuclear export factor Nmd3 joins the 60S pre-ribosome at the level of Arx1 (Ydr101c, termed Arx1 for  associated with  ribosomal e xport complex), which could be the trigger for the acquisition of export competence.	gene_phenotype
69849	2	333449	6	NULL	NULL	0	NULL	Nmd3	GP		bind					60S pre-ribosome	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_embo_21_20_5539_s_180	12374754	The nuclear export factor Nmd3 joins the 60S pre-ribosome at the level of Arx1 (Ydr101c, termed Arx1 for  associated with  ribosomal e xport complex), which could be the trigger for the acquisition of export competence.	gene_phenotype
69850	3	333449	6	NULL	NULL	NULL	NULL	statement 2	Process		occurs at the 					Arx1	GP	level of 			NULL		NULL	NULL	NULL	NULL	gw60_embo_21_20_5539_s_180	12374754	The nuclear export factor Nmd3 joins the 60S pre-ribosome at the level of Arx1 (Ydr101c, termed Arx1 for  associated with  ribosomal e xport complex), which could be the trigger for the acquisition of export competence.	gene_phenotype
69851	1	333452	6	NULL	NULL	NULL	NULL	ERV14	GP		encode			YGL054C		COPII vesicle coat protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_genetics_163_3_875_s_165	12663529	ERV14 (YGL054C) and  ERV41 (YNL067C) encode COPII vesicle coat proteins involved in endoplasmic reticulum (ER)-to-Golgi trafficking ( O TTE et al. 2001   ), and both show toxin resistance.	gene_phenotype
69852	2	333452	6	NULL	NULL	NULL	NULL	ERV41	GP		encodes			YNL067C		COPII vesicle coat protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_genetics_163_3_875_s_165	12663529	ERV14 (YGL054C) and  ERV41 (YNL067C) encode COPII vesicle coat proteins involved in endoplasmic reticulum (ER)-to-Golgi trafficking ( O TTE et al. 2001   ), and both show toxin resistance.	gene_phenotype
69853	3	333452	6	NULL	NULL	NULL	NULL	COPII vesicle coat proteins	GP		is involved in					ER to Golgi trafficking	Process				NULL		NULL	NULL	NULL	NULL	gw60_genetics_163_3_875_s_165	12663529	ERV14 (YGL054C) and  ERV41 (YNL067C) encode COPII vesicle coat proteins involved in endoplasmic reticulum (ER)-to-Golgi trafficking ( O TTE et al. 2001   ), and both show toxin resistance.	gene_phenotype
69854	4	333452	6	NULL	NULL	0	NULL	ERV14	GP		show			YGL054C		toxin	Chemical	resistance to			NULL		0	NULL	NULL	NULL	gw60_genetics_163_3_875_s_165	12663529	ERV14 (YGL054C) and  ERV41 (YNL067C) encode COPII vesicle coat proteins involved in endoplasmic reticulum (ER)-to-Golgi trafficking ( O TTE et al. 2001   ), and both show toxin resistance.	gene_phenotype
69855	1	333454	6	NULL	NULL	0	NULL	Ygl129c	GP		is a type of					ribosomal protein	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_19_15861_s_10	11278769	Another newly identified ribosomal protein, Ygl129c, was previously shown to be a member of the DAP-3 family of mitochondrial apoptosis mediators.	gene_phenotype
69856	2	333454	6	NULL	NULL	0	NULL	Ygl129c	GP		is a member of					DAP-3 family of mitochondrial apoptosis mediators	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_19_15861_s_10	11278769	Another newly identified ribosomal protein, Ygl129c, was previously shown to be a member of the DAP-3 family of mitochondrial apoptosis mediators.	gene_phenotype
69857	1	333456	6	NULL	NULL	0	NULL	CRH1	GP		is regulated by					cell cycle	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_9_3245_s_9	10757808	CRH1 and  YLR213c (renamed  CRR1, for  CRH related) were found to be cell cycle regulated and also expressed under sporulation conditions, whereas  CRH2 expression did not vary during the mitotic cycle.	gene_phenotype
69858	2	333456	6	NULL	NULL	0	NULL	YLR213c	GP		is					CRR1	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_9_3245_s_9	10757808	CRH1 and  YLR213c (renamed  CRR1, for  CRH related) were found to be cell cycle regulated and also expressed under sporulation conditions, whereas  CRH2 expression did not vary during the mitotic cycle.	gene_phenotype
69859	3	333456	6	NULL	NULL	0	NULL	YLR213c	GP		is regulated by					cell cycle	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_9_3245_s_9	10757808	CRH1 and  YLR213c (renamed  CRR1, for  CRH related) were found to be cell cycle regulated and also expressed under sporulation conditions, whereas  CRH2 expression did not vary during the mitotic cycle.	gene_phenotype
69860	4	333456	6	NULL	NULL	NULL	NULL	CRH2	GP	expression of	does not vary					mitotic cycle	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_9_3245_s_9	10757808	CRH1 and  YLR213c (renamed  CRR1, for  CRH related) were found to be cell cycle regulated and also expressed under sporulation conditions, whereas  CRH2 expression did not vary during the mitotic cycle.	gene_phenotype
70068	1	333458	6	NULL	NULL	0	NULL	YOL091w product	GP		plays a role in					sporulation	Process				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_yeast_14_4_9559547_s_11	9559547	Disruption of YOR322c causes osmotically  sensitive growth on YEPD at 37 degrees C and the product of YOL091w appears  to play a role in sporulation since the homozygous diploid disruptant  has lost the ability to sporulate.	gene_phenotype
70070	2	333458	6	NULL	NULL	0	NULL	YOR322c	GP	homozygous mutant	does not					sporulate	Process				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_yeast_14_4_9559547_s_11	9559547	Disruption of YOR322c causes osmotically  sensitive growth on YEPD at 37 degrees C and the product of YOL091w appears  to play a role in sporulation since the homozygous diploid disruptant  has lost the ability to sporulate.	gene_phenotype
69893	1	333464	6	NULL	NULL	0	NULL	YBL091C-A ORF	GP	deletion of	silences					telomere	Chromosome				NULL		0	NULL	NULL	NULL	gw60_genetics_158_1_145_s_152	11333225	Furthermore, a strain with a deletion of the YBL091C-A ORF and an  scs2 mutation has approximately the same telomeric silencing defect as the single  scs2delta mutant ( Fig 3).	gene_phenotype
69894	2	333464	6	NULL	NULL	0	NULL	scs2	GP	deletion of	silences					telomere	Chromosome				NULL		0	NULL	NULL	NULL	gw60_genetics_158_1_145_s_152	11333225	Furthermore, a strain with a deletion of the YBL091C-A ORF and an  scs2 mutation has approximately the same telomeric silencing defect as the single  scs2delta mutant ( Fig 3).	gene_phenotype
69895	3	333464	6	NULL	NULL	0	NULL	scs2delta	GP	mutation of	silences					telomere	Chromosome				NULL		0	NULL	NULL	NULL	gw60_genetics_158_1_145_s_152	11333225	Furthermore, a strain with a deletion of the YBL091C-A ORF and an  scs2 mutation has approximately the same telomeric silencing defect as the single  scs2delta mutant ( Fig 3).	gene_phenotype
69896	1	333465	6	NULL	NULL	NULL	NULL	STE11	GP		is required for					pheromone response	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_13_7508_s_176	9636180	The observation that disruption of the YBR059C and YGR179C genes increased alpha factor sensitivity, combined with previous results ( 30-32) demonstrating that the  STE11 and  STE50 genes are required for pheromone response, indicate that four of the ORF-derived perturbagens originate from genes that play a role in pheromone response.	gene_phenotype
69897	2	333465	6	NULL	NULL	0	NULL	STE50	GP		is required for					pheromone response	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_95_13_7508_s_176	9636180	The observation that disruption of the YBR059C and YGR179C genes increased alpha factor sensitivity, combined with previous results ( 30-32) demonstrating that the  STE11 and  STE50 genes are required for pheromone response, indicate that four of the ORF-derived perturbagens originate from genes that play a role in pheromone response.	gene_phenotype
69898	3	333465	6	NULL	NULL	0	NULL	YBR059C	GP	disruption of	increases					alpha factor	GP	sensitivity of 			NULL		0	NULL	NULL	NULL	gw60_pnas_95_13_7508_s_176	9636180	The observation that disruption of the YBR059C and YGR179C genes increased alpha factor sensitivity, combined with previous results ( 30-32) demonstrating that the  STE11 and  STE50 genes are required for pheromone response, indicate that four of the ORF-derived perturbagens originate from genes that play a role in pheromone response.	gene_phenotype
69899	4	333465	6	NULL	NULL	0	NULL	YGR179C gene	GP	disruption of	increases					alpha factor	GP	sensitivity of			NULL		0	NULL	NULL	NULL	gw60_pnas_95_13_7508_s_176	9636180	The observation that disruption of the YBR059C and YGR179C genes increased alpha factor sensitivity, combined with previous results ( 30-32) demonstrating that the  STE11 and  STE50 genes are required for pheromone response, indicate that four of the ORF-derived perturbagens originate from genes that play a role in pheromone response.	gene_phenotype
69900	1	333466	6	NULL	NULL	0	NULL	YBR265w	GP		is 					TSC10 gene	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_46_30688_s_122	9804843	When this transformant was crossed to a wild-type ( TSC10) haploid and the diploids were sporulated and dissected, all products of meiosis were temperature-resistant, indicating that YBR265w is the wild-type  TSC10 gene.	gene_phenotype
69901	1	333467	6	NULL	NULL	NULL	NULL	FY1679-derived delta ygl194c/delta ygl194c	GP		reduces					sporulation	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_yeast_14_7_9639312_s_4	9639312	A diploid FY1679-derived delta  ygl194c/delta ygl194c homozygous disruptant displayed reduced sporulation.	gene_phenotype
69906	1	333468	6	NULL	NULL	NULL	NULL	YGL194c 3	GP		is sensitive to					brefeldin A	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_306	14587103	YGL194c  3  3  C  Hos2 Histone deacetylase Repression of early sporulation genes Sensitivity to brefeldin A	gene_phenotype
69907	2	333468	6	NULL	NULL	0	NULL	Hos2 	GP		is sensitive to					brefeldin A	Chemical				NULL		0	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_306	14587103	YGL194c  3  3  C  Hos2 Histone deacetylase Repression of early sporulation genes Sensitivity to brefeldin A	gene_phenotype
69914	1	333471	6	NULL	NULL	NULL	NULL	YJL112w	GP	mutant	displays					mitochondria morphology	CellComponent	defects in			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_151_2_333_s_113	11038180	Cells bearing a null-mutation in YJL112w displayed mitochondrial morphology and distribution defects identical to those found in  gag mutant cells (data not shown).	gene_phenotype
69917	2	333471	6	NULL	NULL	0	NULL	gag	GP	mutant	displays					mitochondria distribution	CellComponent	defects in			NULL		0	NULL	NULL	NULL	gw60_cellbiol_151_2_333_s_113	11038180	Cells bearing a null-mutation in YJL112w displayed mitochondrial morphology and distribution defects identical to those found in  gag mutant cells (data not shown).	gene_phenotype
69919	3	333471	6	NULL	NULL	0	NULL	YJL112w	GP	mutant	displays					mitochondria morphology	CellComponent	defects in			NULL		0	NULL	NULL	NULL	gw60_cellbiol_151_2_333_s_113	11038180	Cells bearing a null-mutation in YJL112w displayed mitochondrial morphology and distribution defects identical to those found in  gag mutant cells (data not shown).	gene_phenotype
69921	4	333471	6	NULL	NULL	NULL	NULL	gag	GP	mutant	displays					mitochondria distribution	CellComponent	defects in			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_151_2_333_s_113	11038180	Cells bearing a null-mutation in YJL112w displayed mitochondrial morphology and distribution defects identical to those found in  gag mutant cells (data not shown).	gene_phenotype
69925	1	333472	6	NULL	NULL	NULL	NULL	YLR118c	GP		activates					lysophospholipase	GP				NULL	S. cerevisiae	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_35_31740_s_30	12080046	We now have demonstrated that YLR118c, a  S. cerevisiae open reading frame, encodes an enzyme with both lysophospholipase and acyl-protein thioesterase activity  in vitro.	gene_phenotype
69928	2	333472	6	NULL	NULL	NULL	NULL	YLR118c	GP		activates					acyl-protein thioesterase	GP				NULL	S. cerevisiae	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_35_31740_s_30	12080046	We now have demonstrated that YLR118c, a  S. cerevisiae open reading frame, encodes an enzyme with both lysophospholipase and acyl-protein thioesterase activity  in vitro.	gene_phenotype
69932	1	333473	6	NULL	NULL	NULL	NULL	YLR118C	GP		activates					acyl-protein thioesterase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_35_31740_s_178	12080046	Yeast Strains Bearing a Deletion of the APT1 Gene--  Having established that the protein encoded by YLR118C did indeed have acyl-protein thioesterase activity, we proceeded to create a yeast strain that lacked the APT1 gene to assess further the  in vivo function of Apt1p.	gene_phenotype
69982	1	333477	6	NULL	NULL	NULL	NULL	ynl242w	GP		is defective in					sporulation	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_32_30442_s_196	11382760	The  ynl242w homozygous null strain was found to be defective in sporulation and the gene was named  SPO72.	gene_phenotype
69983	2	333477	6	NULL	NULL	0	NULL	ynl242w	GP		is					SPO72	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_32_30442_s_196	11382760	The  ynl242w homozygous null strain was found to be defective in sporulation and the gene was named  SPO72.	gene_phenotype
69984	1	333478	6	NULL	NULL	0	NULL	ynl242w mutant	GP		is defective in					sporulation	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_32_30442_s_209	11382760	The defect in autophagy seen in the  apg2delta strain explains the previously observed sporulation defect of the  ynl242w mutant ( 29).	gene_phenotype
70073	1	333479	6	NULL	NULL	0	NULL	starvation	Process		induces					autophagy	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_45_42422_s_232	11533052	We have shown recently that YNL242w complemented  apg2, a mutant defective in starvation-induced autophagy ( 42).	gene_phenotype
70074	2	333479	6	NULL	NULL	0	NULL	YNL242w	GP		is defective in					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_45_42422_s_232	11533052	We have shown recently that YNL242w complemented  apg2, a mutant defective in starvation-induced autophagy ( 42).	gene_phenotype
70077	1	333480	6	NULL	NULL	0	NULL	proteins	GP		moved from					cytoplasm	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_32_30442_s_198	11382760	Because our studies suggest a more specific role for the  YNL242w gene product in transport of proteins from the cytoplasm to the vacuole, we will refer to this ORF as  APG2 hereafter in this study.	gene_phenotype
70078	2	333480	6	NULL	NULL	0	NULL	proteins	GP		moved to					vacuoles	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_32_30442_s_198	11382760	Because our studies suggest a more specific role for the  YNL242w gene product in transport of proteins from the cytoplasm to the vacuole, we will refer to this ORF as  APG2 hereafter in this study.	gene_phenotype
70079	3	333480	6	NULL	NULL	0	NULL	statement 2	Process		occurs after					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_32_30442_s_198	11382760	Because our studies suggest a more specific role for the  YNL242w gene product in transport of proteins from the cytoplasm to the vacuole, we will refer to this ORF as  APG2 hereafter in this study.	gene_phenotype
70080	4	333480	6	NULL	NULL	0	NULL	YNL242w	GP		is					APG2	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_32_30442_s_198	11382760	Because our studies suggest a more specific role for the  YNL242w gene product in transport of proteins from the cytoplasm to the vacuole, we will refer to this ORF as  APG2 hereafter in this study.	gene_phenotype
70081	5	333480	6	NULL	NULL	0	NULL	YNL242w	GP		plays a role in					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_32_30442_s_198	11382760	Because our studies suggest a more specific role for the  YNL242w gene product in transport of proteins from the cytoplasm to the vacuole, we will refer to this ORF as  APG2 hereafter in this study.	gene_phenotype
71732	1	333483	6	NULL	NULL	0	NULL	omega -Minus region	CellComponent		determines					fusion protein	GP	localization of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_41_26946_s_88	9756943	Identification of omega -Minus Regions Determining Cellular Localization of the Fusion Proteins-- Our previous study ( 24) has shown that the addition of the most C-terminal 40 amino acids of Yjr151c or Ydr077w to a reporter protein directs the resulting fusion proteins into the cell wall and that the addition of the C-terminal amino acids of Yir039c or Ylr120c directs their fusion proteins to the plasma membrane.	gene_phenotype
71733	2	333483	6	NULL	NULL	0	NULL	fusion protein	GP		is directed to					cell wall	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_41_26946_s_88	9756943	Identification of omega -Minus Regions Determining Cellular Localization of the Fusion Proteins-- Our previous study ( 24) has shown that the addition of the most C-terminal 40 amino acids of Yjr151c or Ydr077w to a reporter protein directs the resulting fusion proteins into the cell wall and that the addition of the C-terminal amino acids of Yir039c or Ylr120c directs their fusion proteins to the plasma membrane.	gene_phenotype
71734	3	333483	6	NULL	NULL	0	NULL				directs			C-terminal 40 amino acids of Yjr151c		statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_41_26946_s_88	9756943	Identification of omega -Minus Regions Determining Cellular Localization of the Fusion Proteins-- Our previous study ( 24) has shown that the addition of the most C-terminal 40 amino acids of Yjr151c or Ydr077w to a reporter protein directs the resulting fusion proteins into the cell wall and that the addition of the C-terminal amino acids of Yir039c or Ylr120c directs their fusion proteins to the plasma membrane.	gene_phenotype
71735	4	333483	6	NULL	NULL	0	NULL				directs			C-terminal 40 amino acids of Ydr077w		statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_41_26946_s_88	9756943	Identification of omega -Minus Regions Determining Cellular Localization of the Fusion Proteins-- Our previous study ( 24) has shown that the addition of the most C-terminal 40 amino acids of Yjr151c or Ydr077w to a reporter protein directs the resulting fusion proteins into the cell wall and that the addition of the C-terminal amino acids of Yir039c or Ylr120c directs their fusion proteins to the plasma membrane.	gene_phenotype
71736	5	333483	6	NULL	NULL	0	NULL	fusion protein	GP		is directed to					plasma membrane	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_41_26946_s_88	9756943	Identification of omega -Minus Regions Determining Cellular Localization of the Fusion Proteins-- Our previous study ( 24) has shown that the addition of the most C-terminal 40 amino acids of Yjr151c or Ydr077w to a reporter protein directs the resulting fusion proteins into the cell wall and that the addition of the C-terminal amino acids of Yir039c or Ylr120c directs their fusion proteins to the plasma membrane.	gene_phenotype
71737	6	333483	6	NULL	NULL	0	NULL				directs			C-terminal amino acids of Yir039c		statement 5					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_41_26946_s_88	9756943	Identification of omega -Minus Regions Determining Cellular Localization of the Fusion Proteins-- Our previous study ( 24) has shown that the addition of the most C-terminal 40 amino acids of Yjr151c or Ydr077w to a reporter protein directs the resulting fusion proteins into the cell wall and that the addition of the C-terminal amino acids of Yir039c or Ylr120c directs their fusion proteins to the plasma membrane.	gene_phenotype
71738	7	333483	6	NULL	NULL	0	NULL				directs			C-terminal amino acids of  Ylr120c		statement 5					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_41_26946_s_88	9756943	Identification of omega -Minus Regions Determining Cellular Localization of the Fusion Proteins-- Our previous study ( 24) has shown that the addition of the most C-terminal 40 amino acids of Yjr151c or Ydr077w to a reporter protein directs the resulting fusion proteins into the cell wall and that the addition of the C-terminal amino acids of Yir039c or Ylr120c directs their fusion proteins to the plasma membrane.	gene_phenotype
71739	1	333485	6	NULL	NULL	0	NULL	YNL072w gene			encodes					RNase H					NULL		0	NULL	NULL	NULL	gw60_febslett_421_1_23_s_108	9462832	The following criteria convinced us that gene YNL072w does indeed encode a RNase H: (i) expression in and purification from  E. coli resulted in a protein which is strongly recognized by an antibody, raised against purified calf thymus RNase HI, and (ii) a yeast strain from whose genome gene YNL072w was deleted showed a significant decrease in total RNase H activity ( Fig. 3).	gene_phenotype
71740	2	333485	6	NULL	NULL	0	NULL	YNL072w gene		deletion of	decreases					RNase H		activity of			NULL		0	NULL	NULL	NULL	gw60_febslett_421_1_23_s_108	9462832	The following criteria convinced us that gene YNL072w does indeed encode a RNase H: (i) expression in and purification from  E. coli resulted in a protein which is strongly recognized by an antibody, raised against purified calf thymus RNase HI, and (ii) a yeast strain from whose genome gene YNL072w was deleted showed a significant decrease in total RNase H activity ( Fig. 3).	gene_phenotype
71741	1	333486	6	NULL	NULL	0	NULL	ORF YNL072w	GP		is located on					chromosome XIV	Chromosome				NULL		0	NULL	NULL	NULL	gw60_febslett_421_1_23_s_63	9462832	When searching the budding yeast genome for homologies with the sequence of the enzymatically active subunit of human RNase HI (Frank et al., in preparation) we found ORF YNL072w on chromosome XIV, which encodes a hypothetical protein of 34.9 kDa.	gene_phenotype
71742	2	333486	6	NULL	NULL	NULL	NULL	statement 1	Process		encodes					hypothetical protein of 34.9 kDa	GP				NULL		NULL	NULL	NULL	NULL	gw60_febslett_421_1_23_s_63	9462832	When searching the budding yeast genome for homologies with the sequence of the enzymatically active subunit of human RNase HI (Frank et al., in preparation) we found ORF YNL072w on chromosome XIV, which encodes a hypothetical protein of 34.9 kDa.	gene_phenotype
71743	1	333488	6	NULL	NULL	0	NULL	AUT7 (YBL078c)	GP		is essential for					autophagy					NULL		0	NULL	NULL	NULL	gw60_embo_17_13_3597_s_101	9649430	AUT7 (YBL078c) is essential for autophagy	gene_phenotype
71744	1	333489	6	NULL	NULL	0	NULL	ORF YBL078c (AUT7)	GP		acts as a 					aut2-1 suppressor	GP	mutant			NULL		0	NULL	NULL	NULL	gw60_embo_17_13_3597_s_83	9649430	Isolation of ORF YBL078c (AUT7), an extragenic suppressor of aut2-1 mutant phenotypes: another gene essential for autophagy	gene_phenotype
71765	1	333491	6	NULL	NULL	0	NULL	 GPI-CWPs Ccw12	GP		contains					133 amino acids	amino acid				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_26_3_239_s_146	12165426	Some proteins, like the very small  but presumably abundant GPI-CWPs Ccw12 and Ydr134c with a predicted unprocessed size  of 133 and 66 amino acids, respectively, and a codon adaptation index of 0.870 and  0.646, respectively, may be used as a means to present mannan to the cell surface  ( Fig. 1).	gene_phenotype
71766	2	333491	6	NULL	NULL	0	NULL	GPI-CWPs Ydr134c	GP		contains					66 amino acids	amino acid				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_26_3_239_s_146	12165426	Some proteins, like the very small  but presumably abundant GPI-CWPs Ccw12 and Ydr134c with a predicted unprocessed size  of 133 and 66 amino acids, respectively, and a codon adaptation index of 0.870 and  0.646, respectively, may be used as a means to present mannan to the cell surface  ( Fig. 1).	gene_phenotype
71767	3	333491	6	NULL	NULL	0	NULL	mannan	chemical		is presented to					cell surface	cell component				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_26_3_239_s_146	12165426	Some proteins, like the very small  but presumably abundant GPI-CWPs Ccw12 and Ydr134c with a predicted unprocessed size  of 133 and 66 amino acids, respectively, and a codon adaptation index of 0.870 and  0.646, respectively, may be used as a means to present mannan to the cell surface  ( Fig. 1).	gene_phenotype
71768	1	333492	6	NULL	NULL	0	NULL	YER130c gene	GP		is activated by					Haa1p	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_36_37973_s_188	15229222	The  YER130c gene was shown to be activated by Haa1p, a transcription factor that also activates the  TPO2 gene encoding the polyamine transport protein (see below) ( ).	gene_phenotype
71769	2	333492	6	NULL	NULL	0	NULL	Haa1p	GP		is a type of					Transcription factor	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_36_37973_s_188	15229222	The  YER130c gene was shown to be activated by Haa1p, a transcription factor that also activates the  TPO2 gene encoding the polyamine transport protein (see below) ( ).	gene_phenotype
71770	3	333492	6	NULL	NULL	0	NULL	TPO2 gene	GP		encodes					polyamine transport protein	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_36_37973_s_188	15229222	The  YER130c gene was shown to be activated by Haa1p, a transcription factor that also activates the  TPO2 gene encoding the polyamine transport protein (see below) ( ).	gene_phenotype
71771	4	333492	6	NULL	NULL	0	NULL	Haa1p	GP		activates					TPO2 gene	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_36_37973_s_188	15229222	The  YER130c gene was shown to be activated by Haa1p, a transcription factor that also activates the  TPO2 gene encoding the polyamine transport protein (see below) ( ).	gene_phenotype
71772	1	333494	6	NULL	NULL	0	NULL	YGL183	GP		is a type of					multicopy plasmid	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_9_3078_s_145	11940665	A multicopy plasmid carrying YGL183c suppresses the  hop2-ts defects in spore formation and viable spore production (Fig.  1B); sporulation efficiency is 5%, and spore viability is 82%.	gene_phenotype
71773	2	333494	6	NULL	NULL	0	NULL	hop2-ts	GP		defects in					spore	organism part	formation of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_9_3078_s_145	11940665	A multicopy plasmid carrying YGL183c suppresses the  hop2-ts defects in spore formation and viable spore production (Fig.  1B); sporulation efficiency is 5%, and spore viability is 82%.	gene_phenotype
71774	3	333494	6	NULL	NULL	0	NULL	hop2-ts	GP		defects in					spore	organism part	viable;; production of 			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_9_3078_s_145	11940665	A multicopy plasmid carrying YGL183c suppresses the  hop2-ts defects in spore formation and viable spore production (Fig.  1B); sporulation efficiency is 5%, and spore viability is 82%.	gene_phenotype
71775	1	333496	6	NULL	NULL	NULL	NULL	SPA2 YLL021W Protein	GP		is involved in					cell polarity	process				NULL		NULL	NULL	NULL	NULL	gw70_yeast_22_2_79_s_155	15645503	SPA2  YLL021W Protein involved in cell polarity and cell fusion during mating.	gene_phenotype
71776	2	333496	6	NULL	NULL	0	NULL	SPA2 YLL021W Protein	GP		is involved in					cell fusion	process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_155	15645503	SPA2  YLL021W Protein involved in cell polarity and cell fusion during mating.	gene_phenotype
71777	1	333497	6	NULL	NULL	0	NULL	FUS1	GP		is induced by					pheromone	chemical				NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_70	10657304	Genes labeled in the plots include previously identified ( FUS1,  FIG1) and novel ( YML047C,  YPL192C) pheromone-induced genes and mitotic cell cycle S phase-induced genes ( HHF1, histone H4, and  RNR1, ribonucleotide reductase large subunit).	gene_phenotype
71778	2	333497	6	NULL	NULL	0	NULL	FIG1	GP		is induced by					pheromone	chemical				NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_70	10657304	Genes labeled in the plots include previously identified ( FUS1,  FIG1) and novel ( YML047C,  YPL192C) pheromone-induced genes and mitotic cell cycle S phase-induced genes ( HHF1, histone H4, and  RNR1, ribonucleotide reductase large subunit).	gene_phenotype
71779	3	333497	6	NULL	NULL	0	NULL	YML047C	GP		is induced by					pheromone	chemical				NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_70	10657304	Genes labeled in the plots include previously identified ( FUS1,  FIG1) and novel ( YML047C,  YPL192C) pheromone-induced genes and mitotic cell cycle S phase-induced genes ( HHF1, histone H4, and  RNR1, ribonucleotide reductase large subunit).	gene_phenotype
71780	4	333497	6	NULL	NULL	0	NULL	YPL192C	GP		is induced by					pheromone	chemical				NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_70	10657304	Genes labeled in the plots include previously identified ( FUS1,  FIG1) and novel ( YML047C,  YPL192C) pheromone-induced genes and mitotic cell cycle S phase-induced genes ( HHF1, histone H4, and  RNR1, ribonucleotide reductase large subunit).	gene_phenotype
71781	5	333497	6	NULL	NULL	NULL	NULL	HHF1	GP		is induced by					 mitotic cell cycle S phase	process				NULL		NULL	NULL	NULL	NULL	gw60_science_287_5454_873_s_70	10657304	Genes labeled in the plots include previously identified ( FUS1,  FIG1) and novel ( YML047C,  YPL192C) pheromone-induced genes and mitotic cell cycle S phase-induced genes ( HHF1, histone H4, and  RNR1, ribonucleotide reductase large subunit).	gene_phenotype
71782	6	333497	6	NULL	NULL	NULL	NULL	histone H4	GP		is induced by					mitotic cell cycle S phase	process				NULL		NULL	NULL	NULL	NULL	gw60_science_287_5454_873_s_70	10657304	Genes labeled in the plots include previously identified ( FUS1,  FIG1) and novel ( YML047C,  YPL192C) pheromone-induced genes and mitotic cell cycle S phase-induced genes ( HHF1, histone H4, and  RNR1, ribonucleotide reductase large subunit).	gene_phenotype
71783	7	333497	6	NULL	NULL	0	NULL	RNR1	GP		is induced by					mitotic cell cycle S phase	process				NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_70	10657304	Genes labeled in the plots include previously identified ( FUS1,  FIG1) and novel ( YML047C,  YPL192C) pheromone-induced genes and mitotic cell cycle S phase-induced genes ( HHF1, histone H4, and  RNR1, ribonucleotide reductase large subunit).	gene_phenotype
71784	8	333497	6	NULL	NULL	0	NULL	ribonucleotide reductase large subunit	GP		is induced by					mitotic cell cycle S phase	process				NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_70	10657304	Genes labeled in the plots include previously identified ( FUS1,  FIG1) and novel ( YML047C,  YPL192C) pheromone-induced genes and mitotic cell cycle S phase-induced genes ( HHF1, histone H4, and  RNR1, ribonucleotide reductase large subunit).	gene_phenotype
71785	1	333498	6	NULL	NULL	0	NULL	YML070W/ DAK1	GP		results in					DAK activity	process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_3_1415_s_131	12401799	Overexpression of the  YML070W/ DAK1 gene product in a DAK double deletion strain resulted in a roughly 250-fold enhanced specific DAK activity compared with the wild type to 1040 units/mg protein during growth in basal medium	gene_phenotype
71786	1	333499	6	NULL	NULL	0	NULL	YNL278W	GP	mutant	shows					cell shape	PhysicalPhenomenon	abnormal			NULL		0	NULL	NULL	NULL	gw70_yeast_20_5_407_s_135	12673624	The disruptant of  YNL278W showed abnormal cell shape and abnormal deposition of chitin (Figure  2B).	gene_phenotype
71787	2	333499	6	NULL	NULL	0	NULL	YNL278W	GP	mutant	shows					chitin 	cell component	abnormal;; deposition of 			NULL		0	NULL	NULL	NULL	gw70_yeast_20_5_407_s_135	12673624	The disruptant of  YNL278W showed abnormal cell shape and abnormal deposition of chitin (Figure  2B).	gene_phenotype
71788	1	333500	6	NULL	NULL	0	NULL	Nug1	GP	yeast	is essential for					viability	process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_1_460_s_138	16251348	In contrast, genes encoding similar putative GTPases from yeast,  Nug1 ( YER006W) and  Nug2/Nog2 ( YNR053C; Bassler  et al., 2001 ; Saveanu  et al., 2001 ) were essential for viability.	gene_phenotype
71789	2	333500	6	NULL	NULL	0	NULL	Nug2/Nog2	GP		is essential for					viability	process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_1_460_s_138	16251348	In contrast, genes encoding similar putative GTPases from yeast,  Nug1 ( YER006W) and  Nug2/Nog2 ( YNR053C; Bassler  et al., 2001 ; Saveanu  et al., 2001 ) were essential for viability.	gene_phenotype
71790	1	333501	6	NULL	NULL	0	NULL	Ynr074cp	GP	purified	degrades					nuclei	cell component	yeast			NULL		0	NULL	NULL	NULL	gw70_cellbiol_166_7_969_s_6	15381687	Purified Ynr074cp degrades yeast nuclei and plasmid DNA.  YNR074C disruption rescues yeast cells from oxygen stress and delays age-induced apoptosis.	gene_phenotype
71791	2	333501	6	NULL	NULL	0	NULL	Ynr074cp	GP		degrades					plasmid DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_cellbiol_166_7_969_s_6	15381687	Purified Ynr074cp degrades yeast nuclei and plasmid DNA.  YNR074C disruption rescues yeast cells from oxygen stress and delays age-induced apoptosis.	gene_phenotype
71792	3	333501	6	NULL	NULL	0	NULL	age	PhysicalPhenomenon		induces					apoptosis	process				NULL		0	NULL	NULL	NULL	gw70_cellbiol_166_7_969_s_6	15381687	Purified Ynr074cp degrades yeast nuclei and plasmid DNA.  YNR074C disruption rescues yeast cells from oxygen stress and delays age-induced apoptosis.	gene_phenotype
71793	4	333501	6	NULL	NULL	NULL	NULL	Ynr074cp	GP	disruption of	delays					statement 3	process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_166_7_969_s_6	15381687	Purified Ynr074cp degrades yeast nuclei and plasmid DNA.  YNR074C disruption rescues yeast cells from oxygen stress and delays age-induced apoptosis.	gene_phenotype
71794	5	333501	6	NULL	NULL	0	NULL	oxygen stress	PhysicalPhenomenon		disrupts					yeast cells	Cell				NULL		0	NULL	NULL	NULL	gw70_cellbiol_166_7_969_s_6	15381687	Purified Ynr074cp degrades yeast nuclei and plasmid DNA.  YNR074C disruption rescues yeast cells from oxygen stress and delays age-induced apoptosis.	gene_phenotype
71795	6	333501	6	NULL	NULL	NULL	NULL	Ynr074cp	GP	disruption of	rescues					statement 5	process				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_166_7_969_s_6	15381687	Purified Ynr074cp degrades yeast nuclei and plasmid DNA.  YNR074C disruption rescues yeast cells from oxygen stress and delays age-induced apoptosis.	gene_phenotype
71796	1	333503	6	NULL	NULL	0	NULL	Ynr074cp	GP		is homologous to					AIF	GP				NULL		0	NULL	NULL	NULL	gw70_cellbiol_166_7_969_s_4	15381687	Here, we show that the yeast AIF homologue Ynr074cp controls yeast apoptosis.	gene_phenotype
71797	2	333503	6	NULL	NULL	0	NULL	Ynr074cp	GP	yeast	controls					apoptosis	process				NULL		0	NULL	NULL	NULL	gw70_cellbiol_166_7_969_s_4	15381687	Here, we show that the yeast AIF homologue Ynr074cp controls yeast apoptosis.	gene_phenotype
71798	1	333504	6	NULL	NULL	0	NULL	AIF	GP		migrate to					nucleus	cell component				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_4_1802_s_257	16436509	We also tried to investigate whether Ndi1p migrate to nucleus, because AIF (possibly its yeast homologue YNR074C, too) does during apoptosis (Susin  et al., 1999 ;	gene_phenotype
71799	2	333504	6	NULL	NULL	0	NULL	statement 1	process		occurs during					apoptosis	process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_4_1802_s_257	16436509	We also tried to investigate whether Ndi1p migrate to nucleus, because AIF (possibly its yeast homologue YNR074C, too) does during apoptosis (Susin  et al., 1999 ;	gene_phenotype
71800	1	333505	6	NULL	NULL	NULL	NULL	Aif1p	GP		translocates from					mitochondria	cell component				NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_166_7_969_s_56	15381687	Aif1p translocates from mitochondria to the nucleus upon apoptosis induction   To determine the cellular localization of Aif1p in yeast cells, we expressed GFP-tagged Ynr074cp (Aif1pyEGFP).	gene_phenotype
71801	2	333505	6	NULL	NULL	0	NULL	Aif1p	GP		translocates to					nucleus	cell component				NULL		0	NULL	NULL	NULL	gw70_cellbiol_166_7_969_s_56	15381687	Aif1p translocates from mitochondria to the nucleus upon apoptosis induction   To determine the cellular localization of Aif1p in yeast cells, we expressed GFP-tagged Ynr074cp (Aif1pyEGFP).	gene_phenotype
71802	3	333505	6	NULL	NULL	0	NULL	statement 1	process		occurs upon					apoptosis	process	induction of 			NULL		0	NULL	NULL	NULL	gw70_cellbiol_166_7_969_s_56	15381687	Aif1p translocates from mitochondria to the nucleus upon apoptosis induction   To determine the cellular localization of Aif1p in yeast cells, we expressed GFP-tagged Ynr074cp (Aif1pyEGFP).	gene_phenotype
71803	4	333505	6	NULL	NULL	0	NULL	statement 2	process		occurs upon					apoptosis	process	induction of 			NULL		0	NULL	NULL	NULL	gw70_cellbiol_166_7_969_s_56	15381687	Aif1p translocates from mitochondria to the nucleus upon apoptosis induction   To determine the cellular localization of Aif1p in yeast cells, we expressed GFP-tagged Ynr074cp (Aif1pyEGFP).	gene_phenotype
71808	1	333507	6	NULL	NULL	NULL	NULL	Nse1p	GP		bind					Rhc18p	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_24_21585_s_114	11927594	Nse1p Forms a Large Complex with Rhc18p and Yol034wp-- To identify proteins associating with Nse1p in budding yeast cells, we attempted to immunopurify complexes containing Nse1p.	gene_phenotype
71809	2	333507	6	NULL	NULL	0	NULL	Nse1p	GP		bind					Yo1034wp	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_24_21585_s_114	11927594	Nse1p Forms a Large Complex with Rhc18p and Yol034wp-- To identify proteins associating with Nse1p in budding yeast cells, we attempted to immunopurify complexes containing Nse1p.	gene_phenotype
71810	3	333507	6	NULL	NULL	NULL	NULL	statement 1	process		occurs simultaneously with					statement 2	process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_24_21585_s_114	11927594	Nse1p Forms a Large Complex with Rhc18p and Yol034wp-- To identify proteins associating with Nse1p in budding yeast cells, we attempted to immunopurify complexes containing Nse1p.	gene_phenotype
71811	1	333509	6	NULL	NULL	0	NULL	CDC53			has sequence homology with					cullins					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_25_22828_s_129	12676951	The Budding Yeast S. cerevisiae Genome Contains Four Cullin  Genes -- CDC53, CUL3 (ORF YGR003w),  CUL8 (ORF YJL047c), and a  more distant relative,  APC2, which shares only limited sequence  homology with cullins ( Fig.  1 A).	gene_phenotype
71812	2	333509	6	NULL	NULL	0	NULL	CUL3 (ORF YGR003w)			has sequence homology with					cullins					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_25_22828_s_129	12676951	The Budding Yeast S. cerevisiae Genome Contains Four Cullin  Genes -- CDC53, CUL3 (ORF YGR003w),  CUL8 (ORF YJL047c), and a  more distant relative,  APC2, which shares only limited sequence  homology with cullins ( Fig.  1 A).	gene_phenotype
71813	3	333509	6	NULL	NULL	0	NULL	CUL8 (ORF YJL047c)			has sequence homology with					cullins					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_25_22828_s_129	12676951	The Budding Yeast S. cerevisiae Genome Contains Four Cullin  Genes -- CDC53, CUL3 (ORF YGR003w),  CUL8 (ORF YJL047c), and a  more distant relative,  APC2, which shares only limited sequence  homology with cullins ( Fig.  1 A).	gene_phenotype
71814	4	333509	6	NULL	NULL	0	NULL	APC2			has sequence homology with					cullins					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_25_22828_s_129	12676951	The Budding Yeast S. cerevisiae Genome Contains Four Cullin  Genes -- CDC53, CUL3 (ORF YGR003w),  CUL8 (ORF YJL047c), and a  more distant relative,  APC2, which shares only limited sequence  homology with cullins ( Fig.  1 A).	gene_phenotype
71815	1	333511	6	NULL	NULL	0	NULL	YBR016w	GP	polarized distribution of	involves					endocytosis					NULL		0	NULL	NULL	NULL	gw60_currbiol_13_18_1636_s_80	13678596	(B) The polarized distribution of YBR016w involves endocytosis.	gene_phenotype
71816	1	333512	6	NULL	NULL	0	NULL	Fth1	GP		is required for					endocytosis	process	normal;; liquid phase			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_11_4676_s_191	14593073	These Fks1-interacting proteins include Fth1, a protein required for normal fluid phase endocytosis (Wiederkehr  et al., 2001 ); Srv2, a protein involved in actin organization and internalization (Wesp  et al., 1997 ); Ygl051w, a protein that interacts with the endocytic protein Pan1 (Wendland  et al., 1996 ; Poirey  et al., 2002 ); Lcb2, a protein required for receptor internalization that is in involved in the production of sphingoid bases and in activation of the Pkh kinases (Zanolari  et al., 2000 ; Friant  et al., 2001 ); and Stt4, a PI-4 kinase that contributes to localization of Rom2 (Audhya  et al., 2000 ; Audhya and Emr, 2002 ).	gene_phenotype
71817	2	333512	6	NULL	NULL	0	NULL	Srv2	GP		is involved in					actin	cell component	organization of 			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_11_4676_s_191	14593073	These Fks1-interacting proteins include Fth1, a protein required for normal fluid phase endocytosis (Wiederkehr  et al., 2001 ); Srv2, a protein involved in actin organization and internalization (Wesp  et al., 1997 ); Ygl051w, a protein that interacts with the endocytic protein Pan1 (Wendland  et al., 1996 ; Poirey  et al., 2002 ); Lcb2, a protein required for receptor internalization that is in involved in the production of sphingoid bases and in activation of the Pkh kinases (Zanolari  et al., 2000 ; Friant  et al., 2001 ); and Stt4, a PI-4 kinase that contributes to localization of Rom2 (Audhya  et al., 2000 ; Audhya and Emr, 2002 ).	gene_phenotype
71818	3	333512	6	NULL	NULL	0	NULL	Srv2	GP		is involved in					actin	cell component	internalization of 			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_11_4676_s_191	14593073	These Fks1-interacting proteins include Fth1, a protein required for normal fluid phase endocytosis (Wiederkehr  et al., 2001 ); Srv2, a protein involved in actin organization and internalization (Wesp  et al., 1997 ); Ygl051w, a protein that interacts with the endocytic protein Pan1 (Wendland  et al., 1996 ; Poirey  et al., 2002 ); Lcb2, a protein required for receptor internalization that is in involved in the production of sphingoid bases and in activation of the Pkh kinases (Zanolari  et al., 2000 ; Friant  et al., 2001 ); and Stt4, a PI-4 kinase that contributes to localization of Rom2 (Audhya  et al., 2000 ; Audhya and Emr, 2002 ).	gene_phenotype
71819	4	333512	6	NULL	NULL	0	NULL	Srv2	GP		bind					Pan1	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_11_4676_s_191	14593073	These Fks1-interacting proteins include Fth1, a protein required for normal fluid phase endocytosis (Wiederkehr  et al., 2001 ); Srv2, a protein involved in actin organization and internalization (Wesp  et al., 1997 ); Ygl051w, a protein that interacts with the endocytic protein Pan1 (Wendland  et al., 1996 ; Poirey  et al., 2002 ); Lcb2, a protein required for receptor internalization that is in involved in the production of sphingoid bases and in activation of the Pkh kinases (Zanolari  et al., 2000 ; Friant  et al., 2001 ); and Stt4, a PI-4 kinase that contributes to localization of Rom2 (Audhya  et al., 2000 ; Audhya and Emr, 2002 ).	gene_phenotype
71820	5	333512	6	NULL	NULL	0	NULL	Lcb2	GP		is required for					receptor	GP	internalization of 			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_11_4676_s_191	14593073	These Fks1-interacting proteins include Fth1, a protein required for normal fluid phase endocytosis (Wiederkehr  et al., 2001 ); Srv2, a protein involved in actin organization and internalization (Wesp  et al., 1997 ); Ygl051w, a protein that interacts with the endocytic protein Pan1 (Wendland  et al., 1996 ; Poirey  et al., 2002 ); Lcb2, a protein required for receptor internalization that is in involved in the production of sphingoid bases and in activation of the Pkh kinases (Zanolari  et al., 2000 ; Friant  et al., 2001 ); and Stt4, a PI-4 kinase that contributes to localization of Rom2 (Audhya  et al., 2000 ; Audhya and Emr, 2002 ).	gene_phenotype
71821	6	333512	6	NULL	NULL	0	NULL	Lcb2	GP		is involved in					sphingoid bases	chemical	production of 			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_11_4676_s_191	14593073	These Fks1-interacting proteins include Fth1, a protein required for normal fluid phase endocytosis (Wiederkehr  et al., 2001 ); Srv2, a protein involved in actin organization and internalization (Wesp  et al., 1997 ); Ygl051w, a protein that interacts with the endocytic protein Pan1 (Wendland  et al., 1996 ; Poirey  et al., 2002 ); Lcb2, a protein required for receptor internalization that is in involved in the production of sphingoid bases and in activation of the Pkh kinases (Zanolari  et al., 2000 ; Friant  et al., 2001 ); and Stt4, a PI-4 kinase that contributes to localization of Rom2 (Audhya  et al., 2000 ; Audhya and Emr, 2002 ).	gene_phenotype
71822	7	333512	6	NULL	NULL	0	NULL	Lcb2	GP		is required for					Pkh kinase	GP	activation of 			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_11_4676_s_191	14593073	These Fks1-interacting proteins include Fth1, a protein required for normal fluid phase endocytosis (Wiederkehr  et al., 2001 ); Srv2, a protein involved in actin organization and internalization (Wesp  et al., 1997 ); Ygl051w, a protein that interacts with the endocytic protein Pan1 (Wendland  et al., 1996 ; Poirey  et al., 2002 ); Lcb2, a protein required for receptor internalization that is in involved in the production of sphingoid bases and in activation of the Pkh kinases (Zanolari  et al., 2000 ; Friant  et al., 2001 ); and Stt4, a PI-4 kinase that contributes to localization of Rom2 (Audhya  et al., 2000 ; Audhya and Emr, 2002 ).	gene_phenotype
71823	8	333512	6	NULL	NULL	0	NULL	Stt4	GP		is a type of					PI-4 kinase	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_11_4676_s_191	14593073	These Fks1-interacting proteins include Fth1, a protein required for normal fluid phase endocytosis (Wiederkehr  et al., 2001 ); Srv2, a protein involved in actin organization and internalization (Wesp  et al., 1997 ); Ygl051w, a protein that interacts with the endocytic protein Pan1 (Wendland  et al., 1996 ; Poirey  et al., 2002 ); Lcb2, a protein required for receptor internalization that is in involved in the production of sphingoid bases and in activation of the Pkh kinases (Zanolari  et al., 2000 ; Friant  et al., 2001 ); and Stt4, a PI-4 kinase that contributes to localization of Rom2 (Audhya  et al., 2000 ; Audhya and Emr, 2002 ).	gene_phenotype
71824	9	333512	6	NULL	NULL	0	NULL	Stt4	GP		contributes to					Rom2	GP	localization of 			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_11_4676_s_191	14593073	These Fks1-interacting proteins include Fth1, a protein required for normal fluid phase endocytosis (Wiederkehr  et al., 2001 ); Srv2, a protein involved in actin organization and internalization (Wesp  et al., 1997 ); Ygl051w, a protein that interacts with the endocytic protein Pan1 (Wendland  et al., 1996 ; Poirey  et al., 2002 ); Lcb2, a protein required for receptor internalization that is in involved in the production of sphingoid bases and in activation of the Pkh kinases (Zanolari  et al., 2000 ; Friant  et al., 2001 ); and Stt4, a PI-4 kinase that contributes to localization of Rom2 (Audhya  et al., 2000 ; Audhya and Emr, 2002 ).	gene_phenotype
71825	1	333513	6	NULL	NULL	NULL	NULL	YJR110w	GP	yeast	encodes					myotubularin-like protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_16_8910_s_142	10900271	Budding yeast contain a single ORF (YJR110w) that encodes a myotubularin-like protein ( 5,  8).	gene_phenotype
71826	1	333514	6	NULL	NULL	0	NULL	YJR110w	GP	recombinant	possesses					PI(3)P phosphatase activity	process				NULL		0	NULL	NULL	NULL	gw60_pnas_97_16_8910_s_144	10900271	In addition, we have found that a recombinant YJR110w fusion protein possesses  in vitro PI(3)P phosphatase activity comparable to that of myotubularin (data not shown).	gene_phenotype
71827	1	333515	6	NULL	NULL	0	NULL	YMR1	GP		is					myotubularin-related gene	GP				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_70_0_247_s_421	11395408	Consistent with these observations, a null mutant strain of budding yeast in which  the myotubularin-related gene  YMR1 (YJR110w) is deleted exhibits increased PI(3)P levels compared to wild-type yeast  ( 138).	gene_phenotype
71828	2	333515	6	NULL	NULL	0	NULL	YJR110w	GP		increases					PI(3)P 	GP	levels of 			NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_70_0_247_s_421	11395408	Consistent with these observations, a null mutant strain of budding yeast in which  the myotubularin-related gene  YMR1 (YJR110w) is deleted exhibits increased PI(3)P levels compared to wild-type yeast  ( 138).	gene_phenotype
71829	1	333517	6	NULL	NULL	0	NULL	calcineurin	GP		is required for					cell wall	organism part				NULL		0	NULL	NULL	NULL	gw60_embo_19_14_3618_s_185	10899116	Calcineurin mutations are synthetically lethal with  vph6 or  fks1 mutations (because calcineurin is required for cell wall biosynthesis or cation homeostasis in such mutants), whereas  ykl159c vph6 and  ykl159c fks1 double mutants were viable (not shown).	gene_phenotype
71830	2	333517	6	NULL	NULL	0	NULL	calcineurin	GP		is required for					cation homeostasis	process				NULL		0	NULL	NULL	NULL	gw60_embo_19_14_3618_s_185	10899116	Calcineurin mutations are synthetically lethal with  vph6 or  fks1 mutations (because calcineurin is required for cell wall biosynthesis or cation homeostasis in such mutants), whereas  ykl159c vph6 and  ykl159c fks1 double mutants were viable (not shown).	gene_phenotype
71831	1	333518	6	NULL	NULL	NULL	NULL	YKL159c	GP		is a homolog of					CBP1	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_19_14_3618_s_39	10899116	Saccharomyces cerevisiae mutants lacking the CBP1 homolog YKL159c were viable and sensitive to cation stress, similar to calcineurin mutants.	gene_phenotype
71832	1	333520	6	NULL	NULL	0	NULL	APG17 YLR423c	GP		is required for					Apg1 protein kinase	GP	activation of 			NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_268	15334557	APG17   YLR423c Required for activation of Apg1 protein kinase; autophagy pathway	gene_phenotype
71835	1	333522	6	NULL	NULL	0	NULL	Ykt6p	GP		is involved in					 endoplasmic reticulum-Golgi transport	process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24323_s_188	15044472	In addition, two other proteins were identified: Ykt6p, a protein involved in endoplasmic reticulum-Golgi transport, and YOR051C, an uncharacterized protein associated with the nuclear pore complex ( ).	gene_phenotype
71836	2	333522	6	NULL	NULL	0	NULL	YOR051C	GP		is associated with					nuclear pore complex	cell component				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24323_s_188	15044472	In addition, two other proteins were identified: Ykt6p, a protein involved in endoplasmic reticulum-Golgi transport, and YOR051C, an uncharacterized protein associated with the nuclear pore complex ( ).	gene_phenotype
71840	1	333524	6	NULL	NULL	0	NULL	SPS2	GP		is not essential for					sporulation	process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_5_3259_s_205	16672465	Homozygous haploid null  SPS2 and  YCL048w mutants of  S. cerevisiae sporulate as efficiently as wild-type strains with normal spore viability, suggesting that these genes are not essential for sporulation ( ,  ).	gene_phenotype
71841	2	333524	6	NULL	NULL	NULL	NULL	YCL048w	GP		is not essential for					sporulation	process				NULL		NULL	NULL	NULL	NULL	gw70_applenvironmicrob_72_5_3259_s_205	16672465	Homozygous haploid null  SPS2 and  YCL048w mutants of  S. cerevisiae sporulate as efficiently as wild-type strains with normal spore viability, suggesting that these genes are not essential for sporulation ( ,  ).	gene_phenotype
71837	1	333525	6	NULL	NULL	0	NULL	YCL048w/ SPS2	GP	homozygous;; mutant	produces					spores	organism part	blebbed			NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_5_3259_s_206	16672465	However, the  YCL048w/ SPS2 homozygous diploid null mutant produced aberrant, blebbed spores surrounded by abnormal cell walls ( ), showing that these two  ECM33 homologs indeed play essential roles in ascospore formation.	gene_phenotype
71838	2	333525	6	NULL	NULL	0	NULL	YCL048w/ SPS2	GP	homozygous;; mutant	is surrounded by					cell wall	cell component	abnormal			NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_5_3259_s_206	16672465	However, the  YCL048w/ SPS2 homozygous diploid null mutant produced aberrant, blebbed spores surrounded by abnormal cell walls ( ), showing that these two  ECM33 homologs indeed play essential roles in ascospore formation.	gene_phenotype
71839	3	333525	6	NULL	NULL	0	NULL	YCL048w/ SPS2	GP		plays a role in					ascospore	cell component	formation of			NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_5_3259_s_206	16672465	However, the  YCL048w/ SPS2 homozygous diploid null mutant produced aberrant, blebbed spores surrounded by abnormal cell walls ( ), showing that these two  ECM33 homologs indeed play essential roles in ascospore formation.	gene_phenotype
68151	1	333526	11	NULL	NULL	0	NULL	Ecm33p	GP		is associate with					sporulation	Process				NULL	S. cerevisiae	0	NULL	NULL	NULL	gw70_applenvironmicrob_72_5_3259_s_139	16672465	In  S. cerevisiae, Ecm33p belongs to a family which contains four members that are separated into two clusters (Sps2p and YCL048wp; Pst1p and Ecm33p) and that are associated with a sporulation function, at least for the first cluster (A. M. Neiman, personal communication;  ).	gene_phenotype
68152	2	333526	11	NULL	NULL	0	NULL	Pst1p	GP		is associate with					sporulation	Process				NULL	S. cerevisiae	0	NULL	NULL	NULL	gw70_applenvironmicrob_72_5_3259_s_139	16672465	In  S. cerevisiae, Ecm33p belongs to a family which contains four members that are separated into two clusters (Sps2p and YCL048wp; Pst1p and Ecm33p) and that are associated with a sporulation function, at least for the first cluster (A. M. Neiman, personal communication;  ).	gene_phenotype
68153	3	333526	11	NULL	NULL	0	NULL	YCL048wp	GP		is associate with					sporulation	Process				NULL	S. cerevisiae	0	NULL	NULL	NULL	gw70_applenvironmicrob_72_5_3259_s_139	16672465	In  S. cerevisiae, Ecm33p belongs to a family which contains four members that are separated into two clusters (Sps2p and YCL048wp; Pst1p and Ecm33p) and that are associated with a sporulation function, at least for the first cluster (A. M. Neiman, personal communication;  ).	gene_phenotype
68154	4	333526	11	NULL	NULL	0	NULL	Sps2p	GP		is associate with					sporulation	Process				NULL	S. cerevisiae	0	NULL	NULL	NULL	gw70_applenvironmicrob_72_5_3259_s_139	16672465	In  S. cerevisiae, Ecm33p belongs to a family which contains four members that are separated into two clusters (Sps2p and YCL048wp; Pst1p and Ecm33p) and that are associated with a sporulation function, at least for the first cluster (A. M. Neiman, personal communication;  ).	gene_phenotype
68155	1	333527	11	NULL	NULL	0	NULL	FEN2	GP	mutant	is					YCR028c	GP				NULL	mitochondrial	0	NULL	NULL	NULL	gw70_genetics_166_2_707_s_314	15020461	However,  FEN2 (YCR028c) was listed in a table of mitochondrial mutants that showed a reduction in cell size.	gene_phenotype
68156	2	333527	11	NULL	NULL	0	NULL	FEN2	GP		shows					reduction in cell size	Process				NULL	mitochondrial	0	NULL	NULL	NULL	gw70_genetics_166_2_707_s_314	15020461	However,  FEN2 (YCR028c) was listed in a table of mitochondrial mutants that showed a reduction in cell size.	gene_phenotype
68157	1	333528	11	NULL	NULL	0	NULL	YCR028c	GP		binds					Single-stranded DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_147	15334557	RIM1   YCR028c Single-stranded DNA-binding protein; essential for mitochondrial genome maintenance	gene_phenotype
68158	2	333528	11	NULL	NULL	0	NULL	YCR028c	GP		is essential for					genome maintenance	Process	mitochondrial			NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_147	15334557	RIM1   YCR028c Single-stranded DNA-binding protein; essential for mitochondrial genome maintenance	gene_phenotype
68159	1	333530	11	NULL	NULL	NULL	NULL	YDR205W	NucleicAcid	S. cerevisiae	is the locus name of					MSC2 protein	GP	S. cerevisiae			NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_27_2_313_s_390	12829273	A third  S. cerevisiae protein, MSC2 (YDR205W), is also involved in zinc transport [  ].	gene_phenotype
68160	2	333530	11	NULL	NULL	NULL	NULL	statement 1	GP		is involved in 					zinc transport	Process				NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_27_2_313_s_390	12829273	A third  S. cerevisiae protein, MSC2 (YDR205W), is also involved in zinc transport [  ].	gene_phenotype
68161	1	333531	11	NULL	NULL	NULL	NULL	YDR205W	NucleicAcid	 yeast 	is a type of 					membrane protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_7_5036_s_2	11058603	The sequence of the yeast gene YDR205W places it within the family of cation diffusion facilitators: membrane proteins that transport transition metals.	gene_phenotype
68162	2	333531	11	NULL	NULL	NULL	NULL	YDR205W	NucleicAcid	 yeast 	is a type of 					cation diffusion facilitator	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_7_5036_s_2	11058603	The sequence of the yeast gene YDR205W places it within the family of cation diffusion facilitators: membrane proteins that transport transition metals.	gene_phenotype
68163	3	333531	11	NULL	NULL	NULL	NULL	YDR205W	NucleicAcid	 yeast 	transports					transition metals	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_7_5036_s_2	11058603	The sequence of the yeast gene YDR205W places it within the family of cation diffusion facilitators: membrane proteins that transport transition metals.	gene_phenotype
68164	1	333532	11	NULL	NULL	0	NULL	YDR205W	GP	Deletion	 increases					unequal sister chromatid recombination	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_7_5036_s_3	11058603	Deletion of YDR205W was reported to result in an increase in unequal sister chromatid recombination and was named meiotic sister chromatid recombination 2 ( MSC2; Thompson, D.	gene_phenotype
68165	2	333532	11	NULL	NULL	0	NULL	statement 1	Process		is					meiotic sister chromatid recombination 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_7_5036_s_3	11058603	Deletion of YDR205W was reported to result in an increase in unequal sister chromatid recombination and was named meiotic sister chromatid recombination 2 ( MSC2; Thompson, D.	gene_phenotype
68166	3	333532	11	NULL	NULL	NULL	NULL	meiotic sister chromatid recombination 2	Process		is					MSC2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_7_5036_s_3	11058603	Deletion of YDR205W was reported to result in an increase in unequal sister chromatid recombination and was named meiotic sister chromatid recombination 2 ( MSC2; Thompson, D.	gene_phenotype
68167	1	333533	11	10	NULL	NULL	NULL	nhx1delta cells	Cell		secretes					CPY	GP				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_12_4277_s_149	11102523	The secretion of CPY by  nhx1delta cells was therefore due to the loss of Nhx1p rather than the loss of a protein encoded by the YDR455C ORF.	gene_phenotype
68168	2	333533	11	NULL	NULL	0	NULL	Nhx1p	GP	 loss of	leads to					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_12_4277_s_149	11102523	The secretion of CPY by  nhx1delta cells was therefore due to the loss of Nhx1p rather than the loss of a protein encoded by the YDR455C ORF.	gene_phenotype
68644	3	333533	11	NULL	NULL	0	NULL	YDR455C ORF	NucleicAcid	loss of;;protein encoded by	does not lead to					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_12_4277_s_149	11102523	The secretion of CPY by  nhx1delta cells was therefore due to the loss of Nhx1p rather than the loss of a protein encoded by the YDR455C ORF.	gene_phenotype
68169	1	333534	11	NULL	NULL	NULL	NULL	statement 4	NucleicAcid		is required for 					 growth	Process				NULL		NULL	NULL	NULL	NULL	gw70_genomeres_16_3_365_s_194	16510898	YGR271C-A and  YGR272C constitute a contiguous ORF required for growth at 37 degrees C, growth on HU-containing  media and cell cycle progression.	gene_phenotype
68170	2	333534	11	NULL	NULL	NULL	NULL	statement 4	NucleicAcid		is required for 					 growth	Process				NULL	on HU-containing media	NULL	NULL	NULL	NULL	gw70_genomeres_16_3_365_s_194	16510898	YGR271C-A and  YGR272C constitute a contiguous ORF required for growth at 37 degrees C, growth on HU-containing  media and cell cycle progression.	gene_phenotype
68171	3	333534	11	NULL	NULL	NULL	NULL	statement 4	NucleicAcid		is required for 					cell cycle progression	Process				NULL		NULL	NULL	NULL	NULL	gw70_genomeres_16_3_365_s_194	16510898	YGR271C-A and  YGR272C constitute a contiguous ORF required for growth at 37 degrees C, growth on HU-containing  media and cell cycle progression.	gene_phenotype
68643	4	333534	11	NULL	NULL	0	NULL	YGR271C-A ORF	NucleicAcid		is contiguous to					YGR272C ORF	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_genomeres_16_3_365_s_194	16510898	YGR271C-A and  YGR272C constitute a contiguous ORF required for growth at 37 degrees C, growth on HU-containing  media and cell cycle progression.	gene_phenotype
68175	1	333535	11	NULL	NULL	NULL	NULL	YGR272c ORF	NucleicAcid	inactivation 	 result in					slower growth rate	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_yeast_16_4_10669875_s_5	10669875	The same analysis also revealed that sporulation  of the ygr272cDelta heterozygous diploid produced two small colonies per  ascus that were also G418-resistant, indicating that the inactivation  of ORF YGR272c could result in a slower growth rate.	gene_phenotype
68404	1	333536	11	NULL	NULL	NULL	NULL	Ynl189w	NucleicAcid		is the locus name of					Srp1	GP				NULL		NULL	NULL	NULL	NULL	gw70_yeast_23_3_159_s_144	16498703	Ynl189w  Srp1  1 Karyopherin   homologue, forms a dimer with karyopherin   Kap95p to mediate import of nuclear proteins; binds the nuclear localization signal  of the substrate during import; may also play a role in regulation of protein degradation  L2H  [ 24]	gene_phenotype
68405	2	333536	11	NULL	NULL	0	NULL	Srp1	GP		is  homologue of					Karyopherin	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_144	16498703	Ynl189w  Srp1  1 Karyopherin   homologue, forms a dimer with karyopherin   Kap95p to mediate import of nuclear proteins; binds the nuclear localization signal  of the substrate during import; may also play a role in regulation of protein degradation  L2H  [ 24]	gene_phenotype
68406	3	333536	11	NULL	NULL	0	NULL	Srp1	GP		dimerise with					Kap95p	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_144	16498703	Ynl189w  Srp1  1 Karyopherin   homologue, forms a dimer with karyopherin   Kap95p to mediate import of nuclear proteins; binds the nuclear localization signal  of the substrate during import; may also play a role in regulation of protein degradation  L2H  [ 24]	gene_phenotype
68407	4	333536	11	NULL	NULL	NULL	NULL	statement 3	GP		import					 nuclear proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_yeast_23_3_159_s_144	16498703	Ynl189w  Srp1  1 Karyopherin   homologue, forms a dimer with karyopherin   Kap95p to mediate import of nuclear proteins; binds the nuclear localization signal  of the substrate during import; may also play a role in regulation of protein degradation  L2H  [ 24]	gene_phenotype
68408	5	333536	11	NULL	NULL	NULL	NULL	Srp1	GP		regulate		may			protein degradation	Process				NULL		NULL	NULL	NULL	NULL	gw70_yeast_23_3_159_s_144	16498703	Ynl189w  Srp1  1 Karyopherin   homologue, forms a dimer with karyopherin   Kap95p to mediate import of nuclear proteins; binds the nuclear localization signal  of the substrate during import; may also play a role in regulation of protein degradation  L2H  [ 24]	gene_phenotype
69243	6	333536	11	NULL	NULL	0	NULL	Kap95p	GP		is a type of 					karyopherin	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_144	16498703	Ynl189w  Srp1  1 Karyopherin   homologue, forms a dimer with karyopherin   Kap95p to mediate import of nuclear proteins; binds the nuclear localization signal  of the substrate during import; may also play a role in regulation of protein degradation  L2H  [ 24]	gene_phenotype
68409	1	333537	11	NULL	NULL	0	NULL	M1 RNA	NucleicAcid		mediate					cleavage	Process				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_21_6920_s_130	16332695	However, in the presence of 40 mM Sr2+ and 0.1 mM Mg2+ we did not observe M1 RNA mediated cleavage (data not shown).	gene_phenotype
68495	1	333539	11	NULL	NULL	0	NULL	Sct1p	GP		is a type of 					choline transporter suppressor	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_45_41710_s_37	11544256	In the present study, we demonstrate that the choline transporter suppressor, Sct1p, encoded by  YBL011w, and a closely related protein encoded by  YKR067w, are two yeast  sn-1 acyltransferases catalyzing both G-3-P and DHAP acylation.	gene_phenotype
68496	2	333539	11	NULL	NULL	NULL	NULL	statement 1	GP		is encoded by					YBL011w	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_41710_s_37	11544256	In the present study, we demonstrate that the choline transporter suppressor, Sct1p, encoded by  YBL011w, and a closely related protein encoded by  YKR067w, are two yeast  sn-1 acyltransferases catalyzing both G-3-P and DHAP acylation.	gene_phenotype
68497	3	333539	11	NULL	NULL	NULL	NULL	statement 1	GP		is a type of 					sn-1 acyltransferases	GP	yeast			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_45_41710_s_37	11544256	In the present study, we demonstrate that the choline transporter suppressor, Sct1p, encoded by  YBL011w, and a closely related protein encoded by  YKR067w, are two yeast  sn-1 acyltransferases catalyzing both G-3-P and DHAP acylation.	gene_phenotype
68498	4	333539	11	NULL	NULL	0	NULL	statement 3	GP		 acylate					G-3-P	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_45_41710_s_37	11544256	In the present study, we demonstrate that the choline transporter suppressor, Sct1p, encoded by  YBL011w, and a closely related protein encoded by  YKR067w, are two yeast  sn-1 acyltransferases catalyzing both G-3-P and DHAP acylation.	gene_phenotype
68499	5	333539	11	NULL	NULL	0	NULL	statement 3	GP		acylate					DHAP	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_45_41710_s_37	11544256	In the present study, we demonstrate that the choline transporter suppressor, Sct1p, encoded by  YBL011w, and a closely related protein encoded by  YKR067w, are two yeast  sn-1 acyltransferases catalyzing both G-3-P and DHAP acylation.	gene_phenotype
68500	1	333540	11	NULL	NULL	NULL	NULL	YBR026c	NucleicAcid		restore					respiratory growth	Process				NULL	ybr026cdelta strain	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_18_6243_s_267	11509667	The complementation experiments with either  YBR026c or  ETR1 showed that either of these genes was sufficient for restoring respiratory growth to the  ybr026cdelta strain (Fig.  4).	gene_phenotype
68501	2	333540	11	NULL	NULL	NULL	NULL	ETR1 gene	GP		restore					respiratory growth	Process	ybr026cdelta strain			NULL	ybr026cdelta strain	NULL	NULL	NULL	NULL	gw60_molcellbiol_21_18_6243_s_267	11509667	The complementation experiments with either  YBR026c or  ETR1 showed that either of these genes was sufficient for restoring respiratory growth to the  ybr026cdelta strain (Fig.  4).	gene_phenotype
68502	1	333541	11	NULL	NULL	NULL	NULL	YOR267c	NucleicAcid		is a type of 					 protein kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_20_7654_s_177	11003661	As indicated above, the protein kinase YOR267c also affected Pma1 activity, although to a lesser extent than Ptk2.	gene_phenotype
68503	2	333541	11	NULL	NULL	NULL	NULL	statement 1	GP		affects					 Pma1	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_20_7654_s_177	11003661	As indicated above, the protein kinase YOR267c also affected Pma1 activity, although to a lesser extent than Ptk2.	gene_phenotype
68504	3	333541	11	NULL	NULL	NULL	NULL	Ptk2	GP		affects					Pma1	GP	activity of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_20_7654_s_177	11003661	As indicated above, the protein kinase YOR267c also affected Pma1 activity, although to a lesser extent than Ptk2.	gene_phenotype
68505	4	333541	11	NULL	NULL	0	NULL	statement 2	Process		is lesser than					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_20_7654_s_177	11003661	As indicated above, the protein kinase YOR267c also affected Pma1 activity, although to a lesser extent than Ptk2.	gene_phenotype
69245	1	333543	11	NULL	NULL	0	NULL	LB	AminoAcid		function as					scilencer-barrier	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	gw60_genetics_160_4_1401_s_209	11973296	Our preliminary deletion analysis indicates that sequences from both the UAS and the ORF of  YCL069W contribute to the silencing-barrier function of LB (X. BI, unpublished results).	gene_phenotype
69246	2	333543	11	NULL	NULL	0	NULL	UAS	NucleicAcid		contribute to					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_160_4_1401_s_209	11973296	Our preliminary deletion analysis indicates that sequences from both the UAS and the ORF of  YCL069W contribute to the silencing-barrier function of LB (X. BI, unpublished results).	gene_phenotype
69247	3	333543	11	NULL	NULL	0	NULL	YCL069W ORF	NucleicAcid		contribute to					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_160_4_1401_s_209	11973296	Our preliminary deletion analysis indicates that sequences from both the UAS and the ORF of  YCL069W contribute to the silencing-barrier function of LB (X. BI, unpublished results).	gene_phenotype
68508	1	333547	11	NULL	NULL	0	NULL	Fcy2p	GP		is a transporter for					 adenine	NucleicAcid				NULL	S. cerevisiae	0	NULL	NULL	NULL	gw70_jbiolchem_278_21_18990_s_121	12649274	The identified ORF, YGL186C, codes for a protein  with homology to Fcy2p, the  S. cerevisiae transporter for adenine,  guanine, and cytosine ( ,  ).	gene_phenotype
68509	2	333547	11	NULL	NULL	0	NULL	Fcy2p	GP		is a transporter for					guanine	NucleicAcid				NULL	S. cerevisiae	0	NULL	NULL	NULL	gw70_jbiolchem_278_21_18990_s_121	12649274	The identified ORF, YGL186C, codes for a protein  with homology to Fcy2p, the  S. cerevisiae transporter for adenine,  guanine, and cytosine ( ,  ).	gene_phenotype
68510	3	333547	11	NULL	NULL	0	NULL	Fcy2p	GP		is a transporter for					 cytosine	NucleicAcid				NULL	S. cerevisiae	0	NULL	NULL	NULL	gw70_jbiolchem_278_21_18990_s_121	12649274	The identified ORF, YGL186C, codes for a protein  with homology to Fcy2p, the  S. cerevisiae transporter for adenine,  guanine, and cytosine ( ,  ).	gene_phenotype
70491	4	333547	11	NULL	NULL	0	NULL	YGL186C	NucleicAcid		is a type of 					ORF	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_21_18990_s_121	12649274	The identified ORF, YGL186C, codes for a protein  with homology to Fcy2p, the  S. cerevisiae transporter for adenine,  guanine, and cytosine ( ,  ).	gene_phenotype
70492	5	333547	11	NULL	NULL	0	NULL	YGL186C protein	GP		is homologous to					Fcy2p	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_21_18990_s_121	12649274	The identified ORF, YGL186C, codes for a protein  with homology to Fcy2p, the  S. cerevisiae transporter for adenine,  guanine, and cytosine ( ,  ).	gene_phenotype
68512	2	333549	11	NULL	NULL	NULL	NULL	 lyso-PC 	Chemical		is					lysophosphatidylcholine	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_biochem-j_387_pt-3_15588229_s_2	15588229	When the yeast protein Ypr140w was expressed in Escherichia coli, a lyso-PC  [lysophosphatidylcholine (1-acylglycerophosphorylcholine)] acyltransferase  activity was found associated with the membranes of the bacteria.	gene_phenotype
69169	3	333549	11	NULL	NULL	NULL	NULL	Ypr140w protein	GP	yeast	is expressed in					Escherichia coli	Organism				NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_biochem-j_387_pt-3_15588229_s_2	15588229	When the yeast protein Ypr140w was expressed in Escherichia coli, a lyso-PC  [lysophosphatidylcholine (1-acylglycerophosphorylcholine)] acyltransferase  activity was found associated with the membranes of the bacteria.	gene_phenotype
70493	4	333549	11	NULL	NULL	0	NULL	1-acylglycerophosphorylcholine	Chemical		is a synonym of					lyso-PC	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_biochem-j_387_pt-3_15588229_s_2	15588229	When the yeast protein Ypr140w was expressed in Escherichia coli, a lyso-PC  [lysophosphatidylcholine (1-acylglycerophosphorylcholine)] acyltransferase  activity was found associated with the membranes of the bacteria.	gene_phenotype
70494	5	333549	11	NULL	NULL	0	NULL	statement 3	GP		activates					lyso- PC acyltransferase	GP				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_biochem-j_387_pt-3_15588229_s_2	15588229	When the yeast protein Ypr140w was expressed in Escherichia coli, a lyso-PC  [lysophosphatidylcholine (1-acylglycerophosphorylcholine)] acyltransferase  activity was found associated with the membranes of the bacteria.	gene_phenotype
70495	6	333549	11	NULL	NULL	0	NULL	statement 5	Process		is associated with					Escherichia coli	Organism	membranes of			NULL		0	NULL	NULL	NULL	abs-batch0517-0529_biochem-j_387_pt-3_15588229_s_2	15588229	When the yeast protein Ypr140w was expressed in Escherichia coli, a lyso-PC  [lysophosphatidylcholine (1-acylglycerophosphorylcholine)] acyltransferase  activity was found associated with the membranes of the bacteria.	gene_phenotype
68513	1	333550	11	NULL	NULL	NULL	NULL	Ycl045cp	NucleicAcid		is a type of 					class I membrane proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_30_11148_s_98	16847257	Ycl045cp has the same predicted topology as Erp1p (they are both class I membrane proteins with a large luminal domain and a short C-terminal cytoplasmic tail), and we suggest that Ycl045cp is also part of the ER-Golgi transport machinery.	gene_phenotype
68514	2	333550	11	NULL	NULL	NULL	NULL	statement 1	GP		contains								large luminal domain;; short C-terminal cytoplasmic tail		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_30_11148_s_98	16847257	Ycl045cp has the same predicted topology as Erp1p (they are both class I membrane proteins with a large luminal domain and a short C-terminal cytoplasmic tail), and we suggest that Ycl045cp is also part of the ER-Golgi transport machinery.	gene_phenotype
68516	4	333550	11	NULL	NULL	0	NULL	Erp1p	GP		is a type of 					class I membrane protein	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_103_30_11148_s_98	16847257	Ycl045cp has the same predicted topology as Erp1p (they are both class I membrane proteins with a large luminal domain and a short C-terminal cytoplasmic tail), and we suggest that Ycl045cp is also part of the ER-Golgi transport machinery.	gene_phenotype
68517	5	333550	11	NULL	NULL	NULL	NULL	statement 4			has a								large luminal domain;; short C-terminal cytoplasmic tail		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_30_11148_s_98	16847257	Ycl045cp has the same predicted topology as Erp1p (they are both class I membrane proteins with a large luminal domain and a short C-terminal cytoplasmic tail), and we suggest that Ycl045cp is also part of the ER-Golgi transport machinery.	gene_phenotype
68519	7	333550	11	NULL	NULL	NULL	NULL	statement 1	GP		is a part of 					transport machinery	Process	ER-Golgi 			NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_30_11148_s_98	16847257	Ycl045cp has the same predicted topology as Erp1p (they are both class I membrane proteins with a large luminal domain and a short C-terminal cytoplasmic tail), and we suggest that Ycl045cp is also part of the ER-Golgi transport machinery.	gene_phenotype
68520	1	333551	11	NULL	NULL	NULL	NULL	Sge1p	GP		is a type of 					multidrug transporter	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_30_11148_s_83	16847257	In particular, overexpression of the multidrug transporter Sge1p ( ), the COPII vesicle transport protein Erp1p ( ), and the functionally unclassified protein Ycl045cp induces hypertolerance to paraquat.	gene_phenotype
68521	2	333551	11	NULL	NULL	0	NULL	Erp1p	GP		is a type of 					COPII vesicle transport protein	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_103_30_11148_s_83	16847257	In particular, overexpression of the multidrug transporter Sge1p ( ), the COPII vesicle transport protein Erp1p ( ), and the functionally unclassified protein Ycl045cp induces hypertolerance to paraquat.	gene_phenotype
68522	3	333551	11	NULL	NULL	NULL	NULL	statement 1	GP	overexpression of	is hypertolerant to 					paraquat	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_30_11148_s_83	16847257	In particular, overexpression of the multidrug transporter Sge1p ( ), the COPII vesicle transport protein Erp1p ( ), and the functionally unclassified protein Ycl045cp induces hypertolerance to paraquat.	gene_phenotype
68523	4	333551	11	NULL	NULL	NULL	NULL	statement 2	GP	overexpression of	is hypertolerant to 					paraquat	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_30_11148_s_83	16847257	In particular, overexpression of the multidrug transporter Sge1p ( ), the COPII vesicle transport protein Erp1p ( ), and the functionally unclassified protein Ycl045cp induces hypertolerance to paraquat.	gene_phenotype
68524	5	333551	11	NULL	NULL	NULL	NULL	Ycl045cp protein		overexpression of	is hypertolerant to 					paraquat	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_30_11148_s_83	16847257	In particular, overexpression of the multidrug transporter Sge1p ( ), the COPII vesicle transport protein Erp1p ( ), and the functionally unclassified protein Ycl045cp induces hypertolerance to paraquat.	gene_phenotype
68525	1	333552	11	NULL	NULL	NULL	NULL	GET1	GP		involved in					Golgi-ER trafficking	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_30_11148_s_99	16847257	Consistent with this proposal, a recent genomewide epistatic miniarray analysis ( ) has identified genetic interactions between  YCL045C and  GET1 (involved in Golgi-ER trafficking),  PMR1 (Ca2+ transport into the Golgi), and  SSH1 (protein translocation into the ER).	gene_phenotype
68526	2	333552	11	NULL	NULL	NULL	NULL	GET1	GP		interacts with 		Genetic			YCL045C	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_30_11148_s_99	16847257	Consistent with this proposal, a recent genomewide epistatic miniarray analysis ( ) has identified genetic interactions between  YCL045C and  GET1 (involved in Golgi-ER trafficking),  PMR1 (Ca2+ transport into the Golgi), and  SSH1 (protein translocation into the ER).	gene_phenotype
68527	3	333552	11	NULL	NULL	NULL	NULL	Ca2+	Chemical		is transported into					golgi	Cell Component				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_30_11148_s_99	16847257	Consistent with this proposal, a recent genomewide epistatic miniarray analysis ( ) has identified genetic interactions between  YCL045C and  GET1 (involved in Golgi-ER trafficking),  PMR1 (Ca2+ transport into the Golgi), and  SSH1 (protein translocation into the ER).	gene_phenotype
68528	4	333552	11	NULL	NULL	NULL	NULL	protein	GP		translocate to					ER	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_30_11148_s_99	16847257	Consistent with this proposal, a recent genomewide epistatic miniarray analysis ( ) has identified genetic interactions between  YCL045C and  GET1 (involved in Golgi-ER trafficking),  PMR1 (Ca2+ transport into the Golgi), and  SSH1 (protein translocation into the ER).	gene_phenotype
70498	6	333552	11	NULL	NULL	0	NULL	PMR1	GP		plays a role in					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_103_30_11148_s_99	16847257	Consistent with this proposal, a recent genomewide epistatic miniarray analysis ( ) has identified genetic interactions between  YCL045C and  GET1 (involved in Golgi-ER trafficking),  PMR1 (Ca2+ transport into the Golgi), and  SSH1 (protein translocation into the ER).	gene_phenotype
70499	7	333552	11	NULL	NULL	0	NULL	SSH1	GP		plays a role in					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_103_30_11148_s_99	16847257	Consistent with this proposal, a recent genomewide epistatic miniarray analysis ( ) has identified genetic interactions between  YCL045C and  GET1 (involved in Golgi-ER trafficking),  PMR1 (Ca2+ transport into the Golgi), and  SSH1 (protein translocation into the ER).	gene_phenotype
70500	8	333552	11	NULL	NULL	0	NULL	PMR1	GP		interacts with 		genetic			SSH1	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_103_30_11148_s_99	16847257	Consistent with this proposal, a recent genomewide epistatic miniarray analysis ( ) has identified genetic interactions between  YCL045C and  GET1 (involved in Golgi-ER trafficking),  PMR1 (Ca2+ transport into the Golgi), and  SSH1 (protein translocation into the ER).	gene_phenotype
68530	1	333555	11	NULL	NULL	NULL	NULL	YGR024c	NucleicAcid		activates		possibly		 	tRNAHis guanylyltransferase	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_23_2889_s_86	14633974	To determine whether ORFs YGR024c and/or YDL076c are required for tRNAHis guanylyltransferase activity, we analyzed the tRNA of strains that lacked each protein.	gene_phenotype
68531	2	333555	11	NULL	NULL	NULL	NULL	YDL076c 	NucleicAcid		activates		possibly			tRNAHis guanylyltransferase 	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_23_2889_s_86	14633974	To determine whether ORFs YGR024c and/or YDL076c are required for tRNAHis guanylyltransferase activity, we analyzed the tRNA of strains that lacked each protein.	gene_phenotype
70496	3	333555	11	NULL	NULL	0	NULL	YGR024c 	NucleicAcid		is a type of 					ORF	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_genesdev_17_23_2889_s_86	14633974	To determine whether ORFs YGR024c and/or YDL076c are required for tRNAHis guanylyltransferase activity, we analyzed the tRNA of strains that lacked each protein.	gene_phenotype
70497	4	333555	11	NULL	NULL	0	NULL	YDL076c 	NucleicAcid		is a type of 					ORF	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_genesdev_17_23_2889_s_86	14633974	To determine whether ORFs YGR024c and/or YDL076c are required for tRNAHis guanylyltransferase activity, we analyzed the tRNA of strains that lacked each protein.	gene_phenotype
68532	1	333556	11	NULL	NULL	NULL	NULL	YDL076c protein	GP		copurifies with								tRNAHis		NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_23_2889_s_214	14633974	One or more of these activities could be stimulated by the protein encoded by ORF YDL076c, which also copurifies with tRNAHis guanylyltransferase activity (see above).	gene_phenotype
70490	2	333556	11	NULL	NULL	0	NULL	YDL076c	NucleicAcid		is a type of 					ORF	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_genesdev_17_23_2889_s_214	14633974	One or more of these activities could be stimulated by the protein encoded by ORF YDL076c, which also copurifies with tRNAHis guanylyltransferase activity (see above).	gene_phenotype
69170	1	333558	11	NULL	NULL	NULL	NULL	Ygr189c	NucleicAcid		is the locus name of					Crh1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_9_3245_s_289	10757808	By means of fusion of the C-terminal domain of each protein to a reporter protein including a secretion signal, alpha-galactosidase, and a hemagglutinin (HA) epitope, these authors showed that Ygr189c (Crh1) and Yel040w (Crh2) fusion proteins were incorporated into the cell wall and released after treatment with laminarinase ( 14).	gene_phenotype
69171	2	333558	11	NULL	NULL	0	NULL	Yel040w	NucleicAcid		is the locus name of					Crh2	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_9_3245_s_289	10757808	By means of fusion of the C-terminal domain of each protein to a reporter protein including a secretion signal, alpha-galactosidase, and a hemagglutinin (HA) epitope, these authors showed that Ygr189c (Crh1) and Yel040w (Crh2) fusion proteins were incorporated into the cell wall and released after treatment with laminarinase ( 14).	gene_phenotype
69172	3	333558	11	NULL	NULL	NULL	NULL	Crh1	GP		is a type of 					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_9_3245_s_289	10757808	By means of fusion of the C-terminal domain of each protein to a reporter protein including a secretion signal, alpha-galactosidase, and a hemagglutinin (HA) epitope, these authors showed that Ygr189c (Crh1) and Yel040w (Crh2) fusion proteins were incorporated into the cell wall and released after treatment with laminarinase ( 14).	gene_phenotype
69173	4	333558	11	NULL	NULL	NULL	NULL	Crh2	GP		is a type of 					fusion protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_9_3245_s_289	10757808	By means of fusion of the C-terminal domain of each protein to a reporter protein including a secretion signal, alpha-galactosidase, and a hemagglutinin (HA) epitope, these authors showed that Ygr189c (Crh1) and Yel040w (Crh2) fusion proteins were incorporated into the cell wall and released after treatment with laminarinase ( 14).	gene_phenotype
69174	5	333558	11	NULL	NULL	NULL	NULL	Crh1	GP		is incorporated into					cell wall	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_9_3245_s_289	10757808	By means of fusion of the C-terminal domain of each protein to a reporter protein including a secretion signal, alpha-galactosidase, and a hemagglutinin (HA) epitope, these authors showed that Ygr189c (Crh1) and Yel040w (Crh2) fusion proteins were incorporated into the cell wall and released after treatment with laminarinase ( 14).	gene_phenotype
69175	6	333558	11	NULL	NULL	NULL	NULL	Crh2	GP		is incorporated into					cell wall	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_9_3245_s_289	10757808	By means of fusion of the C-terminal domain of each protein to a reporter protein including a secretion signal, alpha-galactosidase, and a hemagglutinin (HA) epitope, these authors showed that Ygr189c (Crh1) and Yel040w (Crh2) fusion proteins were incorporated into the cell wall and released after treatment with laminarinase ( 14).	gene_phenotype
69176	7	333558	11	NULL	NULL	NULL	NULL	laminarinase	GP	treatment	releases					Crh1	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_9_3245_s_289	10757808	By means of fusion of the C-terminal domain of each protein to a reporter protein including a secretion signal, alpha-galactosidase, and a hemagglutinin (HA) epitope, these authors showed that Ygr189c (Crh1) and Yel040w (Crh2) fusion proteins were incorporated into the cell wall and released after treatment with laminarinase ( 14).	gene_phenotype
69177	8	333558	11	NULL	NULL	NULL	NULL	laminarinase	GP	treatment	releases					Crh2	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_9_3245_s_289	10757808	By means of fusion of the C-terminal domain of each protein to a reporter protein including a secretion signal, alpha-galactosidase, and a hemagglutinin (HA) epitope, these authors showed that Ygr189c (Crh1) and Yel040w (Crh2) fusion proteins were incorporated into the cell wall and released after treatment with laminarinase ( 14).	gene_phenotype
70843	9	333558	11	NULL	NULL	0	NULL	statement 5	Process		occurs along with					statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_9_3245_s_289	10757808	By means of fusion of the C-terminal domain of each protein to a reporter protein including a secretion signal, alpha-galactosidase, and a hemagglutinin (HA) epitope, these authors showed that Ygr189c (Crh1) and Yel040w (Crh2) fusion proteins were incorporated into the cell wall and released after treatment with laminarinase ( 14).	gene_phenotype
70844	10	333558	11	NULL	NULL	0	NULL	statement 6	Process		occurs along with					statement 8	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_9_3245_s_289	10757808	By means of fusion of the C-terminal domain of each protein to a reporter protein including a secretion signal, alpha-galactosidase, and a hemagglutinin (HA) epitope, these authors showed that Ygr189c (Crh1) and Yel040w (Crh2) fusion proteins were incorporated into the cell wall and released after treatment with laminarinase ( 14).	gene_phenotype
69178	1	333559	11	NULL	NULL	0	NULL	YER062C	NucleicAcid		is the locus name of					Gpp2p	GP				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_182_1_1_s_39	10612722	Biochemical characterisation of the glycerol-3-phosphate phosphatase in  S. cerevisiae clearly linked the salt-induced  YER062C encoded protein (named Gpp2p) to this enzymatic activity and revealed a totally new protein class of small phosphatases [  19].	gene_phenotype
69179	2	333559	11	NULL	NULL	0	NULL	salt	Chemical		induced					statement 1	GP				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_182_1_1_s_39	10612722	Biochemical characterisation of the glycerol-3-phosphate phosphatase in  S. cerevisiae clearly linked the salt-induced  YER062C encoded protein (named Gpp2p) to this enzymatic activity and revealed a totally new protein class of small phosphatases [  19].	gene_phenotype
69180	3	333559	11	NULL	NULL	0	NULL	glycerol-3-phosphate phosphatase	GP	S. cerevisiae	linked to					statement 2	GP				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_182_1_1_s_39	10612722	Biochemical characterisation of the glycerol-3-phosphate phosphatase in  S. cerevisiae clearly linked the salt-induced  YER062C encoded protein (named Gpp2p) to this enzymatic activity and revealed a totally new protein class of small phosphatases [  19].	gene_phenotype
69181	1	333560	11	NULL	NULL	NULL	NULL	Uso1p protein	GP		 involved in					ER-vesicle transport	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_10_4595_s_249	16030260	The protein encoded by YFR016c has 22% similarity over a segment of 108 amino acids residues to Uso1p, a protein involved in ER-vesicle transport.	gene_phenotype
69185	1	333563	11	NULL	NULL	0	NULL	 TPO1	GP		is encoded by					YLL028w	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_6_3265_s_8	9920864	The results indicate that a membrane protein encoded by  YLL028w ( TPO1) is a polyamine transport protein on the vacuolar membrane.	gene_phenotype
69186	2	333563	11	NULL	NULL	NULL	NULL	TPO1	GP		is a type of 					membrane protein 	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_6_3265_s_8	9920864	The results indicate that a membrane protein encoded by  YLL028w ( TPO1) is a polyamine transport protein on the vacuolar membrane.	gene_phenotype
69187	3	333563	11	NULL	NULL	NULL	NULL	TPO1	GP		is a type of 					polyamine transport protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_6_3265_s_8	9920864	The results indicate that a membrane protein encoded by  YLL028w ( TPO1) is a polyamine transport protein on the vacuolar membrane.	gene_phenotype
70845	4	333563	11	NULL	NULL	0	NULL	 TPO1	GP		is present on					vacuolar membrane	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_6_3265_s_8	9920864	The results indicate that a membrane protein encoded by  YLL028w ( TPO1) is a polyamine transport protein on the vacuolar membrane.	gene_phenotype
69191	1	333565	11	NULL	NULL	0	NULL	 transformed cells	Cell		are resistant to 					MGBG	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_6_3265_s_5	9920864	The transformed cells became resistant to MGBG (methylglyoxal bis(guanylhydrazone)) and paraquat, but not Ni2+ and Co2+, suggesting that the protein encoded by  YLL028w is a transport protein specific for polyamines.	gene_phenotype
69192	2	333565	11	NULL	NULL	0	NULL	MGBG	Chemical		is					methylglyoxal bis guanylhydrazone	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_6_3265_s_5	9920864	The transformed cells became resistant to MGBG (methylglyoxal bis(guanylhydrazone)) and paraquat, but not Ni2+ and Co2+, suggesting that the protein encoded by  YLL028w is a transport protein specific for polyamines.	gene_phenotype
69193	3	333565	11	NULL	NULL	0	NULL	transformed cells	Cell		are resistant to 					 paraquat	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_6_3265_s_5	9920864	The transformed cells became resistant to MGBG (methylglyoxal bis(guanylhydrazone)) and paraquat, but not Ni2+ and Co2+, suggesting that the protein encoded by  YLL028w is a transport protein specific for polyamines.	gene_phenotype
69194	4	333565	11	NULL	NULL	0	NULL	transformed cells	Cell		are not resistant to 					Ni2+	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_6_3265_s_5	9920864	The transformed cells became resistant to MGBG (methylglyoxal bis(guanylhydrazone)) and paraquat, but not Ni2+ and Co2+, suggesting that the protein encoded by  YLL028w is a transport protein specific for polyamines.	gene_phenotype
69195	5	333565	11	NULL	NULL	0	NULL	transformed cells	Cell		are not resistant to 					Co2+	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_6_3265_s_5	9920864	The transformed cells became resistant to MGBG (methylglyoxal bis(guanylhydrazone)) and paraquat, but not Ni2+ and Co2+, suggesting that the protein encoded by  YLL028w is a transport protein specific for polyamines.	gene_phenotype
69196	6	333565	11	NULL	NULL	0	NULL	YLL028w	NucleicAcid		encodes for a 					transport protein	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_6_3265_s_5	9920864	The transformed cells became resistant to MGBG (methylglyoxal bis(guanylhydrazone)) and paraquat, but not Ni2+ and Co2+, suggesting that the protein encoded by  YLL028w is a transport protein specific for polyamines.	gene_phenotype
69197	7	333565	11	NULL	NULL	0	NULL	statement 6	GP		is specific for					polyamines	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_6_3265_s_5	9920864	The transformed cells became resistant to MGBG (methylglyoxal bis(guanylhydrazone)) and paraquat, but not Ni2+ and Co2+, suggesting that the protein encoded by  YLL028w is a transport protein specific for polyamines.	gene_phenotype
69198	1	333566	11	NULL	NULL	NULL	NULL	YLL028w	NucleicAcid		is a type of					 membrane protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_6_3265_s_19	9920864	A membrane protein on vacuoles, which catalyzes proton gradient-dependent polyamine (putrescine, spermidine, and spermine) transport ( 18), was encoded by one of the genes ( YLL028w).	gene_phenotype
69199	2	333566	11	NULL	NULL	0	NULL	putrescine	Chemical		is a type of 					polyamine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_6_3265_s_19	9920864	A membrane protein on vacuoles, which catalyzes proton gradient-dependent polyamine (putrescine, spermidine, and spermine) transport ( 18), was encoded by one of the genes ( YLL028w).	gene_phenotype
69200	3	333566	11	NULL	NULL	0	NULL	spermidine	Chemical		is a type of 					polyamine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_6_3265_s_19	9920864	A membrane protein on vacuoles, which catalyzes proton gradient-dependent polyamine (putrescine, spermidine, and spermine) transport ( 18), was encoded by one of the genes ( YLL028w).	gene_phenotype
69201	4	333566	11	NULL	NULL	0	NULL	spermine	Chemical		is a type of 					polyamine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_6_3265_s_19	9920864	A membrane protein on vacuoles, which catalyzes proton gradient-dependent polyamine (putrescine, spermidine, and spermine) transport ( 18), was encoded by one of the genes ( YLL028w).	gene_phenotype
69202	5	333566	11	NULL	NULL	NULL	NULL	putrescine	Chemical	 transport of	is dependent on					proton	Chemical	gradient of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_6_3265_s_19	9920864	A membrane protein on vacuoles, which catalyzes proton gradient-dependent polyamine (putrescine, spermidine, and spermine) transport ( 18), was encoded by one of the genes ( YLL028w).	gene_phenotype
69203	6	333566	11	NULL	NULL	NULL	NULL	spermidine	Chemical	transport of	is dependent on					proton	Chemical	gradient of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_6_3265_s_19	9920864	A membrane protein on vacuoles, which catalyzes proton gradient-dependent polyamine (putrescine, spermidine, and spermine) transport ( 18), was encoded by one of the genes ( YLL028w).	gene_phenotype
69204	7	333566	11	NULL	NULL	NULL	NULL	 spermine	Chemical	transport of	is dependent on					proton	Chemical	gradient of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_6_3265_s_19	9920864	A membrane protein on vacuoles, which catalyzes proton gradient-dependent polyamine (putrescine, spermidine, and spermine) transport ( 18), was encoded by one of the genes ( YLL028w).	gene_phenotype
70846	8	333566	11	NULL	NULL	NULL	NULL	YLL028w	NucleicAcid		catalyzes					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_6_3265_s_19	9920864	A membrane protein on vacuoles, which catalyzes proton gradient-dependent polyamine (putrescine, spermidine, and spermine) transport ( 18), was encoded by one of the genes ( YLL028w).	gene_phenotype
70847	9	333566	11	NULL	NULL	0	NULL	YLL028w	NucleicAcid		catalyzes					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_6_3265_s_19	9920864	A membrane protein on vacuoles, which catalyzes proton gradient-dependent polyamine (putrescine, spermidine, and spermine) transport ( 18), was encoded by one of the genes ( YLL028w).	gene_phenotype
70848	10	333566	11	NULL	NULL	0	NULL	YLL028w	NucleicAcid		catalyzes					statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_6_3265_s_19	9920864	A membrane protein on vacuoles, which catalyzes proton gradient-dependent polyamine (putrescine, spermidine, and spermine) transport ( 18), was encoded by one of the genes ( YLL028w).	gene_phenotype
69205	1	333567	11	NULL	NULL	0	NULL	Ino4p	GP		 interacts with					yeast proteins	GP				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_22_4460_s_195	11071933	beta-Galactosidase activity resulting from two-hybrid interactions between Ino4p and Bck2p, YLR422W and YNR064C     CHO1 expression is regulated by growth phase   The above results indicate that Ino4p interacts with several yeast proteins.	gene_phenotype
69206	2	333567	11	NULL	NULL	0	NULL	Ino4p	GP		interacts with 					Bck2p	GP				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_22_4460_s_195	11071933	beta-Galactosidase activity resulting from two-hybrid interactions between Ino4p and Bck2p, YLR422W and YNR064C     CHO1 expression is regulated by growth phase   The above results indicate that Ino4p interacts with several yeast proteins.	gene_phenotype
69207	3	333567	11	NULL	NULL	0	NULL	YLR422W	GP		interacts with 					YNR064C	GP				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_22_4460_s_195	11071933	beta-Galactosidase activity resulting from two-hybrid interactions between Ino4p and Bck2p, YLR422W and YNR064C     CHO1 expression is regulated by growth phase   The above results indicate that Ino4p interacts with several yeast proteins.	gene_phenotype
69208	4	333567	11	NULL	NULL	NULL	NULL	growth phase	Process		regulates					CHO1	GP	 the expression of 			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_22_4460_s_195	11071933	beta-Galactosidase activity resulting from two-hybrid interactions between Ino4p and Bck2p, YLR422W and YNR064C     CHO1 expression is regulated by growth phase   The above results indicate that Ino4p interacts with several yeast proteins.	gene_phenotype
69209	5	333567	11	NULL	NULL	NULL	NULL	statement 2	Process		activates					beta-Galactosidase	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_22_4460_s_195	11071933	beta-Galactosidase activity resulting from two-hybrid interactions between Ino4p and Bck2p, YLR422W and YNR064C     CHO1 expression is regulated by growth phase   The above results indicate that Ino4p interacts with several yeast proteins.	gene_phenotype
69210	6	333567	11	NULL	NULL	NULL	NULL	statement 3	Process		activates					beta-Galactosidase	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_22_4460_s_195	11071933	beta-Galactosidase activity resulting from two-hybrid interactions between Ino4p and Bck2p, YLR422W and YNR064C     CHO1 expression is regulated by growth phase   The above results indicate that Ino4p interacts with several yeast proteins.	gene_phenotype
69211	1	333568	11	NULL	NULL	0	NULL	YMR159c	NucleicAcid		is essential for					autophagy	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_14_3888_s_70	10406794	Thus, YMR159c turned out to be essential for autophagy.	gene_phenotype
69212	1	333569	11	NULL	NULL	0	NULL	YNR051c	NucleicAcid		encodes for					BRE5	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_406	14587103	YNR051c/BRE5 encodes for a protein with no similarity to other proteins in the data bases;   ynr051c has been recently identified in the Secretion Node by Muren  et al. ([ 2001]) as a Brefeldin-sensitive strain.	gene_phenotype
69213	2	333569	11	NULL	NULL	NULL	NULL	YNR051c	NucleicAcid		is present in					Secretion Node	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_406	14587103	YNR051c/BRE5 encodes for a protein with no similarity to other proteins in the data bases;   ynr051c has been recently identified in the Secretion Node by Muren  et al. ([ 2001]) as a Brefeldin-sensitive strain.	gene_phenotype
70849	3	333569	11	NULL	NULL	0	NULL	YNR051c	NucleicAcid		is a type of 					Brefeldin-sensitive strain	Organism				NULL		0	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_406	14587103	YNR051c/BRE5 encodes for a protein with no similarity to other proteins in the data bases;   ynr051c has been recently identified in the Secretion Node by Muren  et al. ([ 2001]) as a Brefeldin-sensitive strain.	gene_phenotype
69214	1	333570	11	NULL	NULL	0	NULL	 yfr021w	NucleicAcid		is the locus name of					aut10	GP				NULL		0	NULL	NULL	NULL	gw60_febslett_508_1_23_s_75	11707261	aut10  ( yfr021w ) cells are defective in the cvt pathway and autophagy	gene_phenotype
69215	2	333570	11	NULL	NULL	0	NULL	aut10 cells	Cell		are defective in					cvt pathway	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_508_1_23_s_75	11707261	aut10  ( yfr021w ) cells are defective in the cvt pathway and autophagy	gene_phenotype
69216	3	333570	11	NULL	NULL	0	NULL	aut10 cells	Cell		are defective in					 autophagy	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_508_1_23_s_75	11707261	aut10  ( yfr021w ) cells are defective in the cvt pathway and autophagy	gene_phenotype
69217	1	333571	11	NULL	NULL	NULL	NULL	YFR021w 	NucleicAcid		is a type of 					ORF	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_febslett_508_1_23_s_71	11707261	As shown below,  YFR021w is essential for autophagy, we therefore term this open reading frame  AUT10.	gene_phenotype
69218	2	333571	11	NULL	NULL	NULL	NULL	YFR021w ORF	NucleicAcid		is essential for					autophagy	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_508_1_23_s_71	11707261	As shown below,  YFR021w is essential for autophagy, we therefore term this open reading frame  AUT10.	gene_phenotype
70850	3	333571	11	NULL	NULL	0	NULL	YFR021w	NucleicAcid		is a synonym of					AUT10	GP				NULL		0	NULL	NULL	NULL	gw60_febslett_508_1_23_s_71	11707261	As shown below,  YFR021w is essential for autophagy, we therefore term this open reading frame  AUT10.	gene_phenotype
69219	1	333572	11	NULL	NULL	NULL	NULL	YFR021w 	NucleicAcid		is a type of 					ORF	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_12_3821_s_248	11739783	Based on the above-mentioned phenomenon, we decided to examine whether the  S. cerevisiae homolog of  GSA12, the open reading frame  YFR021w, could also be a component in the Cvt/autophagic pathway and pexophagy in this yeast.	gene_phenotype
70851	2	333572	11	NULL	NULL	0	NULL	YFR021w	NucleicAcid	 S. cerevisiae	is a homolog of					GSA12	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_12_3821_s_248	11739783	Based on the above-mentioned phenomenon, we decided to examine whether the  S. cerevisiae homolog of  GSA12, the open reading frame  YFR021w, could also be a component in the Cvt/autophagic pathway and pexophagy in this yeast.	gene_phenotype
70852	3	333572	11	NULL	NULL	0	NULL	YFR021w	NucleicAcid	S. cerevisiae	is a component in		possibly			Cvt/autophagic pathway	Process				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_12_3821_s_248	11739783	Based on the above-mentioned phenomenon, we decided to examine whether the  S. cerevisiae homolog of  GSA12, the open reading frame  YFR021w, could also be a component in the Cvt/autophagic pathway and pexophagy in this yeast.	gene_phenotype
70853	4	333572	11	NULL	NULL	0	NULL	YFR021w	NucleicAcid	S. cerevisiae	is a component in		possibly			pexophagy	Process				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_12_3821_s_248	11739783	Based on the above-mentioned phenomenon, we decided to examine whether the  S. cerevisiae homolog of  GSA12, the open reading frame  YFR021w, could also be a component in the Cvt/autophagic pathway and pexophagy in this yeast.	gene_phenotype
69220	1	333573	11	NULL	NULL	0	NULL	YLR018c	NucleicAcid		is the locus name of					Pom34	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_397	14587103	YLR018c  2  0.5  C  Pom34 Component of the nuclear pore Nuclear-cytoplasmic transport	gene_phenotype
69221	2	333573	11	NULL	NULL	NULL	NULL	Pom34	GP		is a component of					 nuclear pore	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_397	14587103	YLR018c  2  0.5  C  Pom34 Component of the nuclear pore Nuclear-cytoplasmic transport	gene_phenotype
69222	3	333573	11	NULL	NULL	NULL	NULL	statement 2	GP		is essential for					Nuclear-cytoplasmic transport	Process				NULL		NULL	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_397	14587103	YLR018c  2  0.5  C  Pom34 Component of the nuclear pore Nuclear-cytoplasmic transport	gene_phenotype
69223	1	333574	11	NULL	NULL	0	NULL	YLR018c	NucleicAcid		encodes for					Pom34p	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_407	14587103	Finally,  YLR018c encodes Pom34p, a integral membrane protein that forms part of the nuclear pore complex  and is involved in the nuclear cytoplasmic transport (Rout  et al., [ 2000]).	gene_phenotype
69224	2	333574	11	NULL	NULL	0	NULL	Pom34p	GP		is a type of 					integral membrane protein	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_407	14587103	Finally,  YLR018c encodes Pom34p, a integral membrane protein that forms part of the nuclear pore complex  and is involved in the nuclear cytoplasmic transport (Rout  et al., [ 2000]).	gene_phenotype
69225	3	333574	11	NULL	NULL	NULL	NULL	Pom34p	GP		 forms a part of					nuclear pore complex	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_407	14587103	Finally,  YLR018c encodes Pom34p, a integral membrane protein that forms part of the nuclear pore complex  and is involved in the nuclear cytoplasmic transport (Rout  et al., [ 2000]).	gene_phenotype
69226	4	333574	11	NULL	NULL	NULL	NULL	statement 3	GP		 is involved in					nuclear cytoplasmic transport	Process				NULL		NULL	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_407	14587103	Finally,  YLR018c encodes Pom34p, a integral membrane protein that forms part of the nuclear pore complex  and is involved in the nuclear cytoplasmic transport (Rout  et al., [ 2000]).	gene_phenotype
69227	1	333575	11	NULL	NULL	0	NULL	Ylr145w	NucleicAcid		is a component of					RNase MRP	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_12_11352_s_32	15637077	We demonstrate that the Ylr145w protein is indeed a protein component of RNase MRP essential for its activity but is not a component of RNase P.	gene_phenotype
69228	2	333575	11	NULL	NULL	NULL	NULL	statement 1	NucleicAcid		activates					RNase MRP	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_12_11352_s_32	15637077	We demonstrate that the Ylr145w protein is indeed a protein component of RNase MRP essential for its activity but is not a component of RNase P.	gene_phenotype
69229	3	333575	11	NULL	NULL	0	NULL	Ylr145w	NucleicAcid		 is not a component of					RNase P	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_12_11352_s_32	15637077	We demonstrate that the Ylr145w protein is indeed a protein component of RNase MRP essential for its activity but is not a component of RNase P.	gene_phenotype
69322	1	333577	11	NULL	NULL	0	NULL	Epidermal growth factor receptor	GP		undergoes					 internalization	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_6_2_225_s_263	10983971	Epidermal growth factor receptor internalization rate is regulated by negative charges near the SH2 binding site Tyr992.	gene_phenotype
69323	2	333577	11	NULL	NULL	NULL	NULL	statement 1	Process	rate of	 is regulated by					Epidermal growth factor receptor	GP	negative charges near	SH2 binding site Tyr992		NULL		NULL	NULL	NULL	NULL	gw60_molcell_6_2_225_s_263	10983971	Epidermal growth factor receptor internalization rate is regulated by negative charges near the SH2 binding site Tyr992.	gene_phenotype
69230	1	333580	11	NULL	NULL	0	NULL	Vma9p	GP		encoded by					YCL005W-A	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_17_17361_s_6	14970230	The functional significance of these proteins for V-ATPase activity had not been tested, but we show that the protein encoded by  YCL005W-A, which we call Vma9p, is essential for V-ATPase activity in yeast.	gene_phenotype
69231	2	333580	11	NULL	NULL	NULL	NULL	Vma9p	GP		activates					 V-ATPase 	GP				NULL	Yeast	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_17_17361_s_6	14970230	The functional significance of these proteins for V-ATPase activity had not been tested, but we show that the protein encoded by  YCL005W-A, which we call Vma9p, is essential for V-ATPase activity in yeast.	gene_phenotype
69232	1	333581	11	NULL	NULL	0	NULL	 Vma9p	GP		encoded by					YCL005W-A	NucleicAcid				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_279_17_14970230_s_6	14970230	The functional significance of these proteins for V-ATPase  activity had not been tested, but we show that the protein encoded by  YCL005W-A, which we call Vma9p, is essential for V-ATPase activity in  yeast.	gene_phenotype
69234	2	333581	11	NULL	NULL	NULL	NULL	Vma9p	GP		activates					V-ATPase 	GP				NULL	yeast	NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_279_17_14970230_s_6	14970230	The functional significance of these proteins for V-ATPase  activity had not been tested, but we show that the protein encoded by  YCL005W-A, which we call Vma9p, is essential for V-ATPase activity in  yeast.	gene_phenotype
69236	1	333583	11	NULL	NULL	0	NULL	YCR098C ORF	NucleicAcid		is the locus name of					GIT1 gene	GP				NULL		0	NULL	NULL	NULL	gw60_genetics_149_4_1707_s_190	9691030	The  GIT1 gene was originally sequenced as part of the  S. cerevisiae genome sequencing project (this ORF was first labeled as YCR137 but is now YCR098C), but no function was assigned to it other than homology to carbohydrate transport proteins ( S OR et al. 1992   ).	gene_phenotype
69237	2	333583	11	NULL	NULL	NULL	NULL	GIT1 gene	GP		is homologus to					carbohydrate transport protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_genetics_149_4_1707_s_190	9691030	The  GIT1 gene was originally sequenced as part of the  S. cerevisiae genome sequencing project (this ORF was first labeled as YCR137 but is now YCR098C), but no function was assigned to it other than homology to carbohydrate transport proteins ( S OR et al. 1992   ).	gene_phenotype
69238	1	333585	11	NULL	NULL	0	NULL	YER089c	NucleicAcid		is the locus name of					PTC2	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_20_2_157_s_148	12518319	PTC2 (YER089c) encodes one of the five members of the type 2C Ser-Thr phosphatase (PP2C)  family in budding yeast (Stark, [ 1996]).	gene_phenotype
71540	2	333585	11	NULL	NULL	0	NULL	PTC2	GP		is a member of					PP2C family	GP				NULL	budding yeast	0	NULL	NULL	NULL	gw70_yeast_20_2_157_s_148	12518319	PTC2 (YER089c) encodes one of the five members of the type 2C Ser-Thr phosphatase (PP2C)  family in budding yeast (Stark, [ 1996]).	gene_phenotype
71541	3	333585	11	NULL	NULL	0	NULL	PP2C	GP		is					type 2C Ser-Thr phosphatase	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_20_2_157_s_148	12518319	PTC2 (YER089c) encodes one of the five members of the type 2C Ser-Thr phosphatase (PP2C)  family in budding yeast (Stark, [ 1996]).	gene_phenotype
71542	1	333588	11	NULL	NULL	0	NULL	Ykl155c	NucleicAcid		is associated with					Small Ribosomal Subunit of Mitochondria	CellComponent	components of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_19_15861_s_53	11278769	Ykl155c Is Associated with Components of the Small Ribosomal Subunit of Mitochondria-- A yeast strain deleted for  YKL155C was viable but unable to grow on glycerol as the sole carbon source (respiration-deficient; data not shown).	gene_phenotype
69239	1	333589	11	NULL	NULL	0	NULL	VBA1	GP		is					vacuolar basic amino acid transporter	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_6_4851_s_79	15572352	These results suggest that the product of the  YMR088c gene ( VBA1,  vacuolar  basic  amino acid transporter) is required for vacuolar uptake of at least histidine and lysine.	gene_phenotype
69240	2	333589	11	NULL	NULL	NULL	NULL	YMR088c	NucleicAcid		is the locus name of					VBA1	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_6_4851_s_79	15572352	These results suggest that the product of the  YMR088c gene ( VBA1,  vacuolar  basic  amino acid transporter) is required for vacuolar uptake of at least histidine and lysine.	gene_phenotype
69241	3	333589	11	NULL	NULL	NULL	NULL	VBA1	GP		is required for					histidine	amino acid	 vacuolar uptake of 			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_6_4851_s_79	15572352	These results suggest that the product of the  YMR088c gene ( VBA1,  vacuolar  basic  amino acid transporter) is required for vacuolar uptake of at least histidine and lysine.	gene_phenotype
69242	4	333589	11	NULL	NULL	NULL	NULL	VBA1	GP		is required for 					 lysine	amino acid	vacuolar uptake of 			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_6_4851_s_79	15572352	These results suggest that the product of the  YMR088c gene ( VBA1,  vacuolar  basic  amino acid transporter) is required for vacuolar uptake of at least histidine and lysine.	gene_phenotype
69305	1	333590	11	NULL	NULL	0	NULL	VBA1	GP		is					vacuolar basic amino acid transporter 1	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_6_4851_s_3	15572352	ATP-dependent uptake of histidine and lysine by isolated vacuolar membrane vesicles was impaired in  YMR088c, a vacuolar basic amino acid transporter 1 ( VBA1)-deleted strain, whereas uptake of tyrosine or calcium was little affected.	gene_phenotype
69306	2	333590	11	NULL	NULL	0	NULL	 YMR088c	NucleicAcid		is a type of 					a vacuolar basic amino acid transporter 1 deleted strain					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_6_4851_s_3	15572352	ATP-dependent uptake of histidine and lysine by isolated vacuolar membrane vesicles was impaired in  YMR088c, a vacuolar basic amino acid transporter 1 ( VBA1)-deleted strain, whereas uptake of tyrosine or calcium was little affected.	gene_phenotype
69307	3	333590	11	NULL	NULL	NULL	NULL	histidine	AminoAcid		is uptaken by					vacuolar membrane vesicles	Cell Component	isolated			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_6_4851_s_3	15572352	ATP-dependent uptake of histidine and lysine by isolated vacuolar membrane vesicles was impaired in  YMR088c, a vacuolar basic amino acid transporter 1 ( VBA1)-deleted strain, whereas uptake of tyrosine or calcium was little affected.	gene_phenotype
71543	4	333590	11	NULL	NULL	0	NULL	statement 3	Process		is dependent on					ATP	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_6_4851_s_3	15572352	ATP-dependent uptake of histidine and lysine by isolated vacuolar membrane vesicles was impaired in  YMR088c, a vacuolar basic amino acid transporter 1 ( VBA1)-deleted strain, whereas uptake of tyrosine or calcium was little affected.	gene_phenotype
71544	5	333590	11	NULL	NULL	0	NULL	statement 4	Process		is impaired in					YMR088c	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_6_4851_s_3	15572352	ATP-dependent uptake of histidine and lysine by isolated vacuolar membrane vesicles was impaired in  YMR088c, a vacuolar basic amino acid transporter 1 ( VBA1)-deleted strain, whereas uptake of tyrosine or calcium was little affected.	gene_phenotype
71545	6	333590	11	NULL	NULL	0	NULL	 lysine	AminoAcid		is uptaken by					vacuolar membrane vesicles	Cell Component	isolated			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_6_4851_s_3	15572352	ATP-dependent uptake of histidine and lysine by isolated vacuolar membrane vesicles was impaired in  YMR088c, a vacuolar basic amino acid transporter 1 ( VBA1)-deleted strain, whereas uptake of tyrosine or calcium was little affected.	gene_phenotype
71546	7	333590	11	NULL	NULL	NULL	NULL	statement 6	Process		is dependent on					ATP	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_6_4851_s_3	15572352	ATP-dependent uptake of histidine and lysine by isolated vacuolar membrane vesicles was impaired in  YMR088c, a vacuolar basic amino acid transporter 1 ( VBA1)-deleted strain, whereas uptake of tyrosine or calcium was little affected.	gene_phenotype
71547	8	333590	11	NULL	NULL	0	NULL	statement 7	Process		is impaired in					YMR088c	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_6_4851_s_3	15572352	ATP-dependent uptake of histidine and lysine by isolated vacuolar membrane vesicles was impaired in  YMR088c, a vacuolar basic amino acid transporter 1 ( VBA1)-deleted strain, whereas uptake of tyrosine or calcium was little affected.	gene_phenotype
69328	1	333598	11	NULL	NULL	0	NULL	ATG4 gene	GP		participate in					 autophagy	Process				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_fems-yeast-res_5_9_15925308_s_9	15925308	Notably, the genes participating in autophagy (ATG4 and  ATG8), the genes encoding a vacuolar protease (PRB1), vacuolar protease  inhibitors (PAI3, PBI2 and TFS1) and YHR138c (a PBI2 homolog) were up-regulated  in the rns4 mutant.	gene_phenotype
69329	2	333598	11	NULL	NULL	0	NULL	ATG8 gene	GP		participate in					autophagy	Process				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_fems-yeast-res_5_9_15925308_s_9	15925308	Notably, the genes participating in autophagy (ATG4 and  ATG8), the genes encoding a vacuolar protease (PRB1), vacuolar protease  inhibitors (PAI3, PBI2 and TFS1) and YHR138c (a PBI2 homolog) were up-regulated  in the rns4 mutant.	gene_phenotype
69330	3	333598	11	NULL	NULL	0	NULL	PRB1 gene	GP		is a type of 					 vacuolar protease	GP				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_fems-yeast-res_5_9_15925308_s_9	15925308	Notably, the genes participating in autophagy (ATG4 and  ATG8), the genes encoding a vacuolar protease (PRB1), vacuolar protease  inhibitors (PAI3, PBI2 and TFS1) and YHR138c (a PBI2 homolog) were up-regulated  in the rns4 mutant.	gene_phenotype
69331	4	333598	11	NULL	NULL	0	NULL	PAI3	GP		is a type of 					vacuolar protease inhibitor	GP				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_fems-yeast-res_5_9_15925308_s_9	15925308	Notably, the genes participating in autophagy (ATG4 and  ATG8), the genes encoding a vacuolar protease (PRB1), vacuolar protease  inhibitors (PAI3, PBI2 and TFS1) and YHR138c (a PBI2 homolog) were up-regulated  in the rns4 mutant.	gene_phenotype
69332	5	333598	11	NULL	NULL	0	NULL	PBI2	GP		is a type of 					vacuolar protease inhibitor	GP				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_fems-yeast-res_5_9_15925308_s_9	15925308	Notably, the genes participating in autophagy (ATG4 and  ATG8), the genes encoding a vacuolar protease (PRB1), vacuolar protease  inhibitors (PAI3, PBI2 and TFS1) and YHR138c (a PBI2 homolog) were up-regulated  in the rns4 mutant.	gene_phenotype
69333	6	333598	11	NULL	NULL	0	NULL	TFS1	GP		is a type of 					vacuolar protease inhibitor	GP				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_fems-yeast-res_5_9_15925308_s_9	15925308	Notably, the genes participating in autophagy (ATG4 and  ATG8), the genes encoding a vacuolar protease (PRB1), vacuolar protease  inhibitors (PAI3, PBI2 and TFS1) and YHR138c (a PBI2 homolog) were up-regulated  in the rns4 mutant.	gene_phenotype
69334	7	333598	11	NULL	NULL	0	NULL	YHR138c	GP		is homologous to					 PBI2 	GP				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_fems-yeast-res_5_9_15925308_s_9	15925308	Notably, the genes participating in autophagy (ATG4 and  ATG8), the genes encoding a vacuolar protease (PRB1), vacuolar protease  inhibitors (PAI3, PBI2 and TFS1) and YHR138c (a PBI2 homolog) were up-regulated  in the rns4 mutant.	gene_phenotype
69335	8	333598	11	NULL	NULL	0	NULL	rns4	GP	mutant	 up-regulate					ATG4	GP				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_fems-yeast-res_5_9_15925308_s_9	15925308	Notably, the genes participating in autophagy (ATG4 and  ATG8), the genes encoding a vacuolar protease (PRB1), vacuolar protease  inhibitors (PAI3, PBI2 and TFS1) and YHR138c (a PBI2 homolog) were up-regulated  in the rns4 mutant.	gene_phenotype
69336	9	333598	11	NULL	NULL	0	NULL	rns4	GP	mutant	up-regulate					ATG8	GP				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_fems-yeast-res_5_9_15925308_s_9	15925308	Notably, the genes participating in autophagy (ATG4 and  ATG8), the genes encoding a vacuolar protease (PRB1), vacuolar protease  inhibitors (PAI3, PBI2 and TFS1) and YHR138c (a PBI2 homolog) were up-regulated  in the rns4 mutant.	gene_phenotype
69337	10	333598	11	NULL	NULL	0	NULL	rns4 	GP	mutant	 up-regulate					PRB1	GP				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_fems-yeast-res_5_9_15925308_s_9	15925308	Notably, the genes participating in autophagy (ATG4 and  ATG8), the genes encoding a vacuolar protease (PRB1), vacuolar protease  inhibitors (PAI3, PBI2 and TFS1) and YHR138c (a PBI2 homolog) were up-regulated  in the rns4 mutant.	gene_phenotype
69338	11	333598	11	NULL	NULL	0	NULL	rns4	GP	mutant	up-regulate					PAI3	GP				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_fems-yeast-res_5_9_15925308_s_9	15925308	Notably, the genes participating in autophagy (ATG4 and  ATG8), the genes encoding a vacuolar protease (PRB1), vacuolar protease  inhibitors (PAI3, PBI2 and TFS1) and YHR138c (a PBI2 homolog) were up-regulated  in the rns4 mutant.	gene_phenotype
69339	12	333598	11	NULL	NULL	0	NULL	rns4	GP	mutant	up-regulate					PBI2	GP				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_fems-yeast-res_5_9_15925308_s_9	15925308	Notably, the genes participating in autophagy (ATG4 and  ATG8), the genes encoding a vacuolar protease (PRB1), vacuolar protease  inhibitors (PAI3, PBI2 and TFS1) and YHR138c (a PBI2 homolog) were up-regulated  in the rns4 mutant.	gene_phenotype
69340	13	333598	11	NULL	NULL	0	NULL	rns4	GP	mutant	up-regulate					TFS1	GP				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_fems-yeast-res_5_9_15925308_s_9	15925308	Notably, the genes participating in autophagy (ATG4 and  ATG8), the genes encoding a vacuolar protease (PRB1), vacuolar protease  inhibitors (PAI3, PBI2 and TFS1) and YHR138c (a PBI2 homolog) were up-regulated  in the rns4 mutant.	gene_phenotype
69341	14	333598	11	NULL	NULL	0	NULL	rns4	GP	mutant	up-regulate					YHR138c	GP				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_fems-yeast-res_5_9_15925308_s_9	15925308	Notably, the genes participating in autophagy (ATG4 and  ATG8), the genes encoding a vacuolar protease (PRB1), vacuolar protease  inhibitors (PAI3, PBI2 and TFS1) and YHR138c (a PBI2 homolog) were up-regulated  in the rns4 mutant.	gene_phenotype
71745	1	333599	11	NULL	NULL	0	NULL	Bar1p	GP		is a type of					protease	GP				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_16_4741_s_4	10438739	Analysis of the amino-terminal sequences revealed that the 120-kDa mannoprotein is Bar1p, the protease involved in the so-called barrier activity in yeast cells, and that the 45- and 40-kDa mannoproteins are the Kex2-unprocessed and Kex2-processed forms of the gene product of open reading frame (ORF)  YJL158c, an ORF that belongs to the  PIR (protein with internal repeats) family of genes, composed thus far of  PIR1,  PIR2/HSP150, and  PIR3.	gene_phenotype
71746	2	333599	11	NULL	NULL	0	NULL	Bar1p	GP		is involved in					barrier activity	Process				NULL	yeast cells	0	NULL	NULL	NULL	gw60_jbacteriol_181_16_4741_s_4	10438739	Analysis of the amino-terminal sequences revealed that the 120-kDa mannoprotein is Bar1p, the protease involved in the so-called barrier activity in yeast cells, and that the 45- and 40-kDa mannoproteins are the Kex2-unprocessed and Kex2-processed forms of the gene product of open reading frame (ORF)  YJL158c, an ORF that belongs to the  PIR (protein with internal repeats) family of genes, composed thus far of  PIR1,  PIR2/HSP150, and  PIR3.	gene_phenotype
71747	3	333599	11	NULL	NULL	0	NULL	YJL158c	NucleicAcid		is a type of					ORF	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_16_4741_s_4	10438739	Analysis of the amino-terminal sequences revealed that the 120-kDa mannoprotein is Bar1p, the protease involved in the so-called barrier activity in yeast cells, and that the 45- and 40-kDa mannoproteins are the Kex2-unprocessed and Kex2-processed forms of the gene product of open reading frame (ORF)  YJL158c, an ORF that belongs to the  PIR (protein with internal repeats) family of genes, composed thus far of  PIR1,  PIR2/HSP150, and  PIR3.	gene_phenotype
71748	4	333599	11	NULL	NULL	0	NULL	YJL158c	NucleicAcid		is a member of					PIR gene family	GP				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_16_4741_s_4	10438739	Analysis of the amino-terminal sequences revealed that the 120-kDa mannoprotein is Bar1p, the protease involved in the so-called barrier activity in yeast cells, and that the 45- and 40-kDa mannoproteins are the Kex2-unprocessed and Kex2-processed forms of the gene product of open reading frame (ORF)  YJL158c, an ORF that belongs to the  PIR (protein with internal repeats) family of genes, composed thus far of  PIR1,  PIR2/HSP150, and  PIR3.	gene_phenotype
71749	5	333599	11	NULL	NULL	0	NULL	PIR	GP		is					protein with internal repeats	GP				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_16_4741_s_4	10438739	Analysis of the amino-terminal sequences revealed that the 120-kDa mannoprotein is Bar1p, the protease involved in the so-called barrier activity in yeast cells, and that the 45- and 40-kDa mannoproteins are the Kex2-unprocessed and Kex2-processed forms of the gene product of open reading frame (ORF)  YJL158c, an ORF that belongs to the  PIR (protein with internal repeats) family of genes, composed thus far of  PIR1,  PIR2/HSP150, and  PIR3.	gene_phenotype
71750	1	333600	11	NULL	NULL	0	NULL	HGT1	GP		is encoded by					YJL212c	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13259_s_112	10788431	Altogether, the data strongly suggest that the protein encoded by YJL212c (from now on referred to as HGT1, high affinity glutathione transporter 1) is probably the glutathione transporter in the plasma membrane of these cells.	gene_phenotype
71751	2	333600	11	NULL	NULL	0	NULL	YJL212c	NucleicAcid	probably	is a type of					glutathione transporter	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13259_s_112	10788431	Altogether, the data strongly suggest that the protein encoded by YJL212c (from now on referred to as HGT1, high affinity glutathione transporter 1) is probably the glutathione transporter in the plasma membrane of these cells.	gene_phenotype
71752	3	333600	11	NULL	NULL	0	NULL	YJL212c	NucleicAcid		is present on					plasma membrane	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13259_s_112	10788431	Altogether, the data strongly suggest that the protein encoded by YJL212c (from now on referred to as HGT1, high affinity glutathione transporter 1) is probably the glutathione transporter in the plasma membrane of these cells.	gene_phenotype
71753	4	333600	11	NULL	NULL	0	NULL	HGT1	GP		is					high affinity glutathione transporter 1	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13259_s_112	10788431	Altogether, the data strongly suggest that the protein encoded by YJL212c (from now on referred to as HGT1, high affinity glutathione transporter 1) is probably the glutathione transporter in the plasma membrane of these cells.	gene_phenotype
69343	2	333604	11	NULL	NULL	0	NULL	GSH1 	GP	locus	undergoes					disruption	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13259_s_48	10788431	The disruption at the  GSH1 locus was followed by glutathione auxotrophy, while disruption at either the  YPR194c locus or the  PTR2 locus was followed either by uracile prototrophy or resistance to G418, respectively.	gene_phenotype
69344	3	333604	11	NULL	NULL	NULL	NULL	statement 2	Process		followed by					auxotrophy	Process	 glutathione			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_18_13259_s_48	10788431	The disruption at the  GSH1 locus was followed by glutathione auxotrophy, while disruption at either the  YPR194c locus or the  PTR2 locus was followed either by uracile prototrophy or resistance to G418, respectively.	gene_phenotype
69345	4	333604	11	NULL	NULL	0	NULL	YPR194c	NucleicAcid	locus	undergoes					disruption	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13259_s_48	10788431	The disruption at the  GSH1 locus was followed by glutathione auxotrophy, while disruption at either the  YPR194c locus or the  PTR2 locus was followed either by uracile prototrophy or resistance to G418, respectively.	gene_phenotype
69346	5	333604	11	NULL	NULL	0	NULL	PTR2	GP	locus	undergoes					disruption	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13259_s_48	10788431	The disruption at the  GSH1 locus was followed by glutathione auxotrophy, while disruption at either the  YPR194c locus or the  PTR2 locus was followed either by uracile prototrophy or resistance to G418, respectively.	gene_phenotype
69348	6	333604	11	NULL	NULL	0	NULL	statement 4	Process		followed by					prototrophy	Process	uracile			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13259_s_48	10788431	The disruption at the  GSH1 locus was followed by glutathione auxotrophy, while disruption at either the  YPR194c locus or the  PTR2 locus was followed either by uracile prototrophy or resistance to G418, respectively.	gene_phenotype
69349	7	333604	11	NULL	NULL	0	NULL	statement 4	Process		followed by					resistance	Process	 to G418			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13259_s_48	10788431	The disruption at the  GSH1 locus was followed by glutathione auxotrophy, while disruption at either the  YPR194c locus or the  PTR2 locus was followed either by uracile prototrophy or resistance to G418, respectively.	gene_phenotype
69350	8	333604	11	NULL	NULL	0	NULL	statement 5	Process		followed by					prototrophy	Process	uracile			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13259_s_48	10788431	The disruption at the  GSH1 locus was followed by glutathione auxotrophy, while disruption at either the  YPR194c locus or the  PTR2 locus was followed either by uracile prototrophy or resistance to G418, respectively.	gene_phenotype
69351	9	333604	11	NULL	NULL	0	NULL	statement 5	Process		followed by					 resistance	Process	to G418			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13259_s_48	10788431	The disruption at the  GSH1 locus was followed by glutathione auxotrophy, while disruption at either the  YPR194c locus or the  PTR2 locus was followed either by uracile prototrophy or resistance to G418, respectively.	gene_phenotype
71754	1	333605	11	NULL	NULL	0	NULL	YPR194c	NucleicAcid		encodes					oligopeptide transporter protein	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13259_s_237	10788431	Therefore, either  YPR194c indeed encodes an oligopeptide transporter protein that is very closely related to  HGT1, or, more likely, it encodes a glutathione transporter localized into a different organelle.	gene_phenotype
71755	2	333605	11	NULL	NULL	0	NULL	YPR194c	NucleicAcid	closely	is related to					HGT1	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13259_s_237	10788431	Therefore, either  YPR194c indeed encodes an oligopeptide transporter protein that is very closely related to  HGT1, or, more likely, it encodes a glutathione transporter localized into a different organelle.	gene_phenotype
71756	3	333605	11	NULL	NULL	0	NULL	YPR194c	NucleicAcid		encodes					glutathione transporter	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13259_s_237	10788431	Therefore, either  YPR194c indeed encodes an oligopeptide transporter protein that is very closely related to  HGT1, or, more likely, it encodes a glutathione transporter localized into a different organelle.	gene_phenotype
71757	4	333605	11	NULL	NULL	0	NULL	statement 1	Process		is an alternative to 					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13259_s_237	10788431	Therefore, either  YPR194c indeed encodes an oligopeptide transporter protein that is very closely related to  HGT1, or, more likely, it encodes a glutathione transporter localized into a different organelle.	gene_phenotype
69352	1	333606	11	NULL	NULL	0	NULL	YDR384c	NucleicAcid		is the locus name of					ATO3	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_45882_s_30	12966084	Here we characterize a retrograde responsive gene,  ATO3 ( YDR384c), whose elevated expression in rhoo petite cells is largely independent of the  RTG genes.	gene_phenotype
69353	2	333606	11	NULL	NULL	NULL	NULL	ATO3	GP	elevated expression of	is independent of		largely			RTG genes	GP				NULL	rhoo petite cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_45882_s_30	12966084	Here we characterize a retrograde responsive gene,  ATO3 ( YDR384c), whose elevated expression in rhoo petite cells is largely independent of the  RTG genes.	gene_phenotype
69355	1	333607	11	NULL	NULL	NULL	NULL	 RPA	GP		is imported to 					nucleus	Cell Component				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_4_729_s_278	11266464	To examine the effect of Ybr137wp on nuclear import of RPA, the localization of Rpa2p-PrA was examined in wild-type and  YBR137W deletion ( YBR137Wdelta) strains.	gene_phenotype
69356	2	333607	11	NULL	NULL	NULL	NULL	Ybr137wp	NucleicAcid		plays a role in		possibly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_152_4_729_s_278	11266464	To examine the effect of Ybr137wp on nuclear import of RPA, the localization of Rpa2p-PrA was examined in wild-type and  YBR137W deletion ( YBR137Wdelta) strains.	gene_phenotype
69358	1	333610	11	NULL	NULL	0	NULL	YMR110c	NucleicAcid		is a type of 					hypothetical open reading frame	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_genetics_163_1_69_s_21	12586697	MSC7/YHR039c encodes a protein with homology to aldehyde deydrogenases that affects meiotic sister-chromatid recombination ( T HOMPSON and STAHL 1999   ), and  YMR110c is a hypothetical open reading frame that could code for an aldehyde-dehydrogenase-related protein.	gene_phenotype
69359	2	333610	11	10	NULL	NULL	NULL	statement 1	NucleicAcid		code for					aldehyde-dehydrogenase-related protein	GP				NULL		NULL	NULL	NULL	NULL	gw60_genetics_163_1_69_s_21	12586697	MSC7/YHR039c encodes a protein with homology to aldehyde deydrogenases that affects meiotic sister-chromatid recombination ( T HOMPSON and STAHL 1999   ), and  YMR110c is a hypothetical open reading frame that could code for an aldehyde-dehydrogenase-related protein.	gene_phenotype
69360	3	333610	11	NULL	NULL	0	NULL	MSC7/YHR039c	GP		is homologous to					aldehyde deydrogenases	GP				NULL		0	NULL	NULL	NULL	gw60_genetics_163_1_69_s_21	12586697	MSC7/YHR039c encodes a protein with homology to aldehyde deydrogenases that affects meiotic sister-chromatid recombination ( T HOMPSON and STAHL 1999   ), and  YMR110c is a hypothetical open reading frame that could code for an aldehyde-dehydrogenase-related protein.	gene_phenotype
69361	4	333610	11	NULL	NULL	0	NULL	MSC7/YHR039c	GP		affects					meiotic sister-chromatid recombination	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_163_1_69_s_21	12586697	MSC7/YHR039c encodes a protein with homology to aldehyde deydrogenases that affects meiotic sister-chromatid recombination ( T HOMPSON and STAHL 1999   ), and  YMR110c is a hypothetical open reading frame that could code for an aldehyde-dehydrogenase-related protein.	gene_phenotype
69362	1	333614	11	NULL	NULL	0	NULL	YSW1 gene	GP		is a type of 					spore-specific protein	GP				NULL		0	NULL	NULL	NULL	gw70_nature_423_6937_241_s_322	12748633	The protein encoded by YBR184W has not been studied extensively, but expression studies  show that the gene is induced during sporulation 33, and sequence analysis shows that it is similar to the gene  YSW1, which encodes a spore-specific protein.	gene_phenotype
69363	2	333614	11	NULL	NULL	NULL	NULL	YBR184W gene	GP		is induced during					sporulation	Process				NULL		NULL	NULL	NULL	NULL	gw70_nature_423_6937_241_s_322	12748633	The protein encoded by YBR184W has not been studied extensively, but expression studies  show that the gene is induced during sporulation 33, and sequence analysis shows that it is similar to the gene  YSW1, which encodes a spore-specific protein.	gene_phenotype
69364	3	333614	11	NULL	NULL	NULL	NULL	YBR184W gene	GP		is similar to					YSW1 gene	GP				NULL		NULL	NULL	NULL	NULL	gw70_nature_423_6937_241_s_322	12748633	The protein encoded by YBR184W has not been studied extensively, but expression studies  show that the gene is induced during sporulation 33, and sequence analysis shows that it is similar to the gene  YSW1, which encodes a spore-specific protein.	gene_phenotype
69365	1	333615	11	NULL	NULL	NULL	NULL	YGR194c gene	GP		 encodes 					xylulokinase	GP				NULL	Saccharomyces cerevisiae	NULL	NULL	NULL	NULL	gw60_applenvironmicrob_69_1_495_s_426	12514033	The YGR194c ( XKS1) gene encodes the xylulokinase from the budding yeast  Saccharomyces cerevisiae.	gene_phenotype
69366	2	333615	11	NULL	NULL	NULL	NULL	YGR194c gene	GP		 is a synonym of 					 XKS1 gene	GP				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_69_1_495_s_426	12514033	The YGR194c ( XKS1) gene encodes the xylulokinase from the budding yeast  Saccharomyces cerevisiae.	gene_phenotype
69367	1	333618	11	NULL	NULL	NULL	NULL	YGR194c gene	GP		encodes for					xylulokinase	GP				NULL	Saccharomyces cerevisiae	NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_190_1_39_s_207	10981687	J.M. Rodrigez-Pena, V.J. Cid, J. Arroyo and C. Nombela, The YGR194c (XKS1) gene encodes the xylulokinase from the budding yeast  Saccharomyces cerevisiae.	gene_phenotype
69368	2	333618	11	NULL	NULL	NULL	NULL	YGR194c gene	GP		 is a synonym of 					 XKS1 gene	GP				NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_190_1_39_s_207	10981687	J.M. Rodrigez-Pena, V.J. Cid, J. Arroyo and C. Nombela, The YGR194c (XKS1) gene encodes the xylulokinase from the budding yeast  Saccharomyces cerevisiae.	gene_phenotype
71758	1	333621	11	NULL	NULL	0	NULL	YJR070C protein	GP		activates					DOHH	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_103_1_51_s_83	16371467	We isolated the pYEX-4T-1/yDOHH plasmid from a single A7 clone expressing DOHH activity in the form of a 62-kDa GST fusion protein (data not shown) and confirmed the nucleotide sequence of the complete ORF.  YJR070C encodes a protein of 325 aa (36 kDa) with DOHH activity.	gene_phenotype
69373	1	333624	11	NULL	NULL	0	NULL	AUT7  gene	GP		is essential for					 autophagy	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_99_26_16875_s_257	12486219	From the list of LAPs for  YNL101W (Table 8, which is published as supporting information on the PNAS web site), we find several genes involved in autophagy, protein degradation, and transport:  AUT7 (essential for autophagy, appearing six times),  PRE6 and  PUP1 (20S proteasome subunits),  RPT6 (26S proteasome-regulatory subunit),  CLC1 (clathrin light chain),  YPT52	gene_phenotype
69374	2	333624	11	NULL	NULL	0	NULL	CLC1 gene	GP		is a type of 					clathrin light chain	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_99_26_16875_s_257	12486219	From the list of LAPs for  YNL101W (Table 8, which is published as supporting information on the PNAS web site), we find several genes involved in autophagy, protein degradation, and transport:  AUT7 (essential for autophagy, appearing six times),  PRE6 and  PUP1 (20S proteasome subunits),  RPT6 (26S proteasome-regulatory subunit),  CLC1 (clathrin light chain),  YPT52	gene_phenotype
71763	3	333624	11	NULL	NULL	0	NULL	PUP1	GP		is a type of 					20S proteasome subunits	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_99_26_16875_s_257	12486219	From the list of LAPs for  YNL101W (Table 8, which is published as supporting information on the PNAS web site), we find several genes involved in autophagy, protein degradation, and transport:  AUT7 (essential for autophagy, appearing six times),  PRE6 and  PUP1 (20S proteasome subunits),  RPT6 (26S proteasome-regulatory subunit),  CLC1 (clathrin light chain),  YPT52	gene_phenotype
71764	4	333624	11	NULL	NULL	0	NULL	RPT6	GP		is a type of 					26S proteasome-regulatory subunit	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_99_26_16875_s_257	12486219	From the list of LAPs for  YNL101W (Table 8, which is published as supporting information on the PNAS web site), we find several genes involved in autophagy, protein degradation, and transport:  AUT7 (essential for autophagy, appearing six times),  PRE6 and  PUP1 (20S proteasome subunits),  RPT6 (26S proteasome-regulatory subunit),  CLC1 (clathrin light chain),  YPT52	gene_phenotype
69698	1	333627	11	NULL	NULL	0	NULL	SPO70 gene	GP	 intron removal	is activated in					 meiosis	Process				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_8_1700_s_7	10734188	One gene (YGR225W/ SPO70) has an intron whose removal is activated during meiosis under control of the  MER1 gene.	gene_phenotype
69699	2	333627	11	NULL	NULL	0	NULL	statement 1	Process		is controlled by 					MER1 gene	GP				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_8_1700_s_7	10734188	One gene (YGR225W/ SPO70) has an intron whose removal is activated during meiosis under control of the  MER1 gene.	gene_phenotype
69700	3	333627	11	NULL	NULL	0	NULL	YGR225W	NucleicAcid		is the locus name of					SPO70	GP				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_8_1700_s_7	10734188	One gene (YGR225W/ SPO70) has an intron whose removal is activated during meiosis under control of the  MER1 gene.	gene_phenotype
69994	1	333629	11	NULL	NULL	0	NULL	YGR225W	NucleicAcid		undergoes					splicing	Process	meiotic time			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_8_1700_s_186	10734188	We measured splicing of YGR225W/ SPO70 during a meiotic time course using a strain capable of synchronous and efficient meiosis ( 19, 22).	gene_phenotype
70052	2	333630	11	NULL	NULL	0	NULL	 YGR225W	NucleicAcid		is the locus name of					SPO70	GP				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_8_1700_s_187	10734188	During meiosis and sporulation, efficiency of YGR225W/ SPO70 splicing is low but increases, as shown by the increase in the ratio of spliced to unspliced RT - PCR product (Fig.  4A).	gene_phenotype
70053	3	333630	11	NULL	NULL	NULL	NULL	YGR225W	Process	splicing of	is less efficient during 					meiosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_8_1700_s_187	10734188	During meiosis and sporulation, efficiency of YGR225W/ SPO70 splicing is low but increases, as shown by the increase in the ratio of spliced to unspliced RT - PCR product (Fig.  4A).	gene_phenotype
70054	4	333630	11	NULL	NULL	NULL	NULL	YGR225W	Process	splicing of	is less efficient during 					sporulation	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_8_1700_s_187	10734188	During meiosis and sporulation, efficiency of YGR225W/ SPO70 splicing is low but increases, as shown by the increase in the ratio of spliced to unspliced RT - PCR product (Fig.  4A).	gene_phenotype
70055	1	333632	11	NULL	NULL	0	NULL	YGR225W	NucleicAcid		undergoes					Splicing	Process				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_8_1700_s_184	10734188	Splicing of YGR225W/ SPO70 is activated during meiosis by  MER1   or the vast majority of introns tested, splicing took place with approximately equivalent efficiencies under the expression conditions we tested.	gene_phenotype
70056	2	333632	11	NULL	NULL	0	NULL	YGR225W	NucleicAcid		is the locus name of					SPO70	GP				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_8_1700_s_184	10734188	Splicing of YGR225W/ SPO70 is activated during meiosis by  MER1   or the vast majority of introns tested, splicing took place with approximately equivalent efficiencies under the expression conditions we tested.	gene_phenotype
70057	3	333632	11	NULL	NULL	0	NULL	MER1	GP		activates					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_8_1700_s_184	10734188	Splicing of YGR225W/ SPO70 is activated during meiosis by  MER1   or the vast majority of introns tested, splicing took place with approximately equivalent efficiencies under the expression conditions we tested.	gene_phenotype
70058	4	333632	11	NULL	NULL	0	NULL	intron	NucleicAcid		activates					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_8_1700_s_184	10734188	Splicing of YGR225W/ SPO70 is activated during meiosis by  MER1   or the vast majority of introns tested, splicing took place with approximately equivalent efficiencies under the expression conditions we tested.	gene_phenotype
70059	5	333632	11	NULL	NULL	0	NULL	statement 3	Process		happens during					meiosis	Process				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_8_1700_s_184	10734188	Splicing of YGR225W/ SPO70 is activated during meiosis by  MER1   or the vast majority of introns tested, splicing took place with approximately equivalent efficiencies under the expression conditions we tested.	gene_phenotype
70060	1	333633	11	NULL	NULL	0	NULL	Imp2p	GP		is a type of 					transcriptional activator	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_20_13_1085_s_2	14558142	Imp2p (Yil154c) is a transcriptional activator involved in glucose derepression of  the maltose, galactose and raffinose utilization pathways and in resistance to thermal,  oxidative or osmotic stress.	gene_phenotype
70061	2	333633	11	NULL	NULL	0	NULL	Yil154c	NucleicAcid		is the locus name of					Imp2p	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_20_13_1085_s_2	14558142	Imp2p (Yil154c) is a transcriptional activator involved in glucose derepression of  the maltose, galactose and raffinose utilization pathways and in resistance to thermal,  oxidative or osmotic stress.	gene_phenotype
70062	3	333633	11	NULL	NULL	0	NULL	glucose	Chemical		undergoes					derepression	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_13_1085_s_2	14558142	Imp2p (Yil154c) is a transcriptional activator involved in glucose derepression of  the maltose, galactose and raffinose utilization pathways and in resistance to thermal,  oxidative or osmotic stress.	gene_phenotype
70063	4	333633	11	NULL	NULL	0	NULL	statement 3	Process		occurs in 					raffinose utilization pathway	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_13_1085_s_2	14558142	Imp2p (Yil154c) is a transcriptional activator involved in glucose derepression of  the maltose, galactose and raffinose utilization pathways and in resistance to thermal,  oxidative or osmotic stress.	gene_phenotype
70064	5	333633	11	NULL	NULL	0	NULL	statement 3	Process		occurs in 					maltose utilization pathway	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_13_1085_s_2	14558142	Imp2p (Yil154c) is a transcriptional activator involved in glucose derepression of  the maltose, galactose and raffinose utilization pathways and in resistance to thermal,  oxidative or osmotic stress.	gene_phenotype
70065	6	333633	11	NULL	NULL	0	NULL	statement 3	Process		occurs in 					galactose utilization pathway	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_13_1085_s_2	14558142	Imp2p (Yil154c) is a transcriptional activator involved in glucose derepression of  the maltose, galactose and raffinose utilization pathways and in resistance to thermal,  oxidative or osmotic stress.	gene_phenotype
70066	7	333633	11	NULL	NULL	0	NULL	Imp2p	GP		 involved in 					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_13_1085_s_2	14558142	Imp2p (Yil154c) is a transcriptional activator involved in glucose derepression of  the maltose, galactose and raffinose utilization pathways and in resistance to thermal,  oxidative or osmotic stress.	gene_phenotype
70067	1	333637	11	NULL	NULL	0	NULL	ygr231c	NucleicAcid		shows					mannosyl phosphorylation	Process	decrease in			NULL		0	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_379	14587103	It is likely that the drop in mannosyl phosphorylation seen in   ygr231c is, as the shorter lifespan, an indirect effect of an increased oxidative stress  or a decrease in the metabolic efficiency.	gene_phenotype
70069	2	333637	11	NULL	NULL	0	NULL	statement 1	Process		is an indirect effect of					oxidative stress 	Process	 increased			NULL		0	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_379	14587103	It is likely that the drop in mannosyl phosphorylation seen in   ygr231c is, as the shorter lifespan, an indirect effect of an increased oxidative stress  or a decrease in the metabolic efficiency.	gene_phenotype
70071	3	333637	11	NULL	NULL	0	NULL	statement 1	Process		is an indirect effect of					metabolic efficiency	Process	decrease in			NULL		0	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_379	14587103	It is likely that the drop in mannosyl phosphorylation seen in   ygr231c is, as the shorter lifespan, an indirect effect of an increased oxidative stress  or a decrease in the metabolic efficiency.	gene_phenotype
70072	4	333637	11	NULL	NULL	0	NULL	statement 2	Process		is an alternative to 					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_379	14587103	It is likely that the drop in mannosyl phosphorylation seen in   ygr231c is, as the shorter lifespan, an indirect effect of an increased oxidative stress  or a decrease in the metabolic efficiency.	gene_phenotype
70075	1	333638	11	NULL	NULL	NULL	NULL	YJR075w	NucleicAcid		corresponds to					HOC1	GP				NULL		NULL	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_223	14587103	YJR075w corresponds to  HOC1, which encodes a type II membrane protein that associates with several other components  (Mnn9p, Anp1p, Mnn10p, Mnn11p) in the  cis-Golgi to form a complex endowed with  1,6-mannosyltransferase activity (complex II).	gene_phenotype
70076	2	333638	11	NULL	NULL	0	NULL	HOC1	GP		is a type of 					type II membrane protein	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_223	14587103	YJR075w corresponds to  HOC1, which encodes a type II membrane protein that associates with several other components  (Mnn9p, Anp1p, Mnn10p, Mnn11p) in the  cis-Golgi to form a complex endowed with  1,6-mannosyltransferase activity (complex II).	gene_phenotype
70091	3	333638	11	NULL	NULL	0	NULL	HOC1	GP		associates with					Mnn9p	GP				NULL	 cis-Golgi	0	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_223	14587103	YJR075w corresponds to  HOC1, which encodes a type II membrane protein that associates with several other components  (Mnn9p, Anp1p, Mnn10p, Mnn11p) in the  cis-Golgi to form a complex endowed with  1,6-mannosyltransferase activity (complex II).	gene_phenotype
70112	4	333638	11	NULL	NULL	0	NULL	HOC1	GP		associates with					Anp1p	GP				NULL	 cis-Golgi	0	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_223	14587103	YJR075w corresponds to  HOC1, which encodes a type II membrane protein that associates with several other components  (Mnn9p, Anp1p, Mnn10p, Mnn11p) in the  cis-Golgi to form a complex endowed with  1,6-mannosyltransferase activity (complex II).	gene_phenotype
70113	5	333638	11	NULL	NULL	0	NULL	 HOC1	GP		associates with					Mnn10p	GP				NULL	 cis-Golgi	0	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_223	14587103	YJR075w corresponds to  HOC1, which encodes a type II membrane protein that associates with several other components  (Mnn9p, Anp1p, Mnn10p, Mnn11p) in the  cis-Golgi to form a complex endowed with  1,6-mannosyltransferase activity (complex II).	gene_phenotype
70114	6	333638	11	NULL	NULL	0	NULL	HOC1	GP		associates with					Mnn11p	GP				NULL	cis-Golgi	0	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_223	14587103	YJR075w corresponds to  HOC1, which encodes a type II membrane protein that associates with several other components  (Mnn9p, Anp1p, Mnn10p, Mnn11p) in the  cis-Golgi to form a complex endowed with  1,6-mannosyltransferase activity (complex II).	gene_phenotype
70115	7	333638	11	NULL	NULL	0	NULL	statement 3	GP		complex with 					statement 4	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_223	14587103	YJR075w corresponds to  HOC1, which encodes a type II membrane protein that associates with several other components  (Mnn9p, Anp1p, Mnn10p, Mnn11p) in the  cis-Golgi to form a complex endowed with  1,6-mannosyltransferase activity (complex II).	gene_phenotype
70116	8	333638	11	NULL	NULL	0	NULL	statement 5	GP		complex with 					statement 6	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_223	14587103	YJR075w corresponds to  HOC1, which encodes a type II membrane protein that associates with several other components  (Mnn9p, Anp1p, Mnn10p, Mnn11p) in the  cis-Golgi to form a complex endowed with  1,6-mannosyltransferase activity (complex II).	gene_phenotype
70117	9	333638	11	NULL	NULL	0	NULL	statement 7	GP		complex with 					statement 8	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_223	14587103	YJR075w corresponds to  HOC1, which encodes a type II membrane protein that associates with several other components  (Mnn9p, Anp1p, Mnn10p, Mnn11p) in the  cis-Golgi to form a complex endowed with  1,6-mannosyltransferase activity (complex II).	gene_phenotype
70118	10	333638	11	NULL	NULL	0	NULL	statement 7	GP		activates					1,6-mannosyltransferase	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_223	14587103	YJR075w corresponds to  HOC1, which encodes a type II membrane protein that associates with several other components  (Mnn9p, Anp1p, Mnn10p, Mnn11p) in the  cis-Golgi to form a complex endowed with  1,6-mannosyltransferase activity (complex II).	gene_phenotype
70119	11	333638	11	NULL	NULL	0	NULL	statement 8	GP		activates					1,6-mannosyltransferase	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_223	14587103	YJR075w corresponds to  HOC1, which encodes a type II membrane protein that associates with several other components  (Mnn9p, Anp1p, Mnn10p, Mnn11p) in the  cis-Golgi to form a complex endowed with  1,6-mannosyltransferase activity (complex II).	gene_phenotype
70120	12	333638	11	NULL	NULL	0	NULL	statement 9	GP		activates					1,6-mannosyltransferase	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_223	14587103	YJR075w corresponds to  HOC1, which encodes a type II membrane protein that associates with several other components  (Mnn9p, Anp1p, Mnn10p, Mnn11p) in the  cis-Golgi to form a complex endowed with  1,6-mannosyltransferase activity (complex II).	gene_phenotype
71843	1	333639	11	NULL	NULL	0	NULL	YMR233W	NucleicAcid		is deleted from					NOY556	Organism	wild type strain			NULL		0	NULL	NULL	NULL	gw60_embo_20_16_4512_s_151	11500378	We found that deletion of  YMR233W from a standard wild-type strain (NOY556) or from a  uaf30 delta strain did not cause any alteration in growth phenotypes, as judged either by colony size (Figure  3A) or by measuring doubling time in YEPD liquid medium (Figure  3B).	gene_phenotype
71844	2	333639	11	NULL	NULL	0	NULL	statement 1	Process		does not alter					growth phenotype	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	gw60_embo_20_16_4512_s_151	11500378	We found that deletion of  YMR233W from a standard wild-type strain (NOY556) or from a  uaf30 delta strain did not cause any alteration in growth phenotypes, as judged either by colony size (Figure  3A) or by measuring doubling time in YEPD liquid medium (Figure  3B).	gene_phenotype
71845	3	333639	11	NULL	NULL	0	NULL	YMR233W	NucleicAcid		is deleted from					uaf30 delta strain	Organism				NULL		0	NULL	NULL	NULL	gw60_embo_20_16_4512_s_151	11500378	We found that deletion of  YMR233W from a standard wild-type strain (NOY556) or from a  uaf30 delta strain did not cause any alteration in growth phenotypes, as judged either by colony size (Figure  3A) or by measuring doubling time in YEPD liquid medium (Figure  3B).	gene_phenotype
71846	4	333639	11	NULL	NULL	0	NULL	statement 3	Process		does not alter					growth phenotype	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	gw60_embo_20_16_4512_s_151	11500378	We found that deletion of  YMR233W from a standard wild-type strain (NOY556) or from a  uaf30 delta strain did not cause any alteration in growth phenotypes, as judged either by colony size (Figure  3A) or by measuring doubling time in YEPD liquid medium (Figure  3B).	gene_phenotype
70124	1	333642	11	NULL	NULL	0	NULL	Cap1 protein	GP	full-length	 less active than					Cap1 protein	GP	truncated			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_31_19304_s_182	9235926	Interestingly, the full-length Cap1 protein was approximately 3 times less active than the truncated Cap1 protein in this assay, indicating that the C-terminal domain of Cap1 behaves as an inhibitor of Cap1 activity with respect to the transcriptional regulation of  YBR008c in  S. cerevisiae (Fig.  6 A).	gene_phenotype
71847	2	333642	11	NULL	NULL	0	NULL	Cap1	GP	C terminal domain of	is an inhibitor of					Cap1 activity	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_31_19304_s_182	9235926	Interestingly, the full-length Cap1 protein was approximately 3 times less active than the truncated Cap1 protein in this assay, indicating that the C-terminal domain of Cap1 behaves as an inhibitor of Cap1 activity with respect to the transcriptional regulation of  YBR008c in  S. cerevisiae (Fig.  6 A).	gene_phenotype
71848	3	333642	11	NULL	NULL	0	NULL	statement 2	Process		with respect to					YBR008c	NucleicAcid	transcriptional regulation of			NULL	S.cerevisiae	0	NULL	NULL	NULL	gw60_jbiolchem_272_31_19304_s_182	9235926	Interestingly, the full-length Cap1 protein was approximately 3 times less active than the truncated Cap1 protein in this assay, indicating that the C-terminal domain of Cap1 behaves as an inhibitor of Cap1 activity with respect to the transcriptional regulation of  YBR008c in  S. cerevisiae (Fig.  6 A).	gene_phenotype
70136	1	333644	11	NULL	NULL	0	NULL	YGL087c ORF	NucleicAcid		 is located on					chromosome VII	Chromosome				NULL	 Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw60_febslett_423_1_49_s_8	9580084	The YGL087c open reading frame of the budding yeast  Saccharomyces cerevisiae is located on chromosome VII  [ 9], encodes a protein with 38% identity to human UEV-1A [ 1, and maintains the same structural features of this class of proteins.	gene_phenotype
70137	1	333645	11	NULL	NULL	0	NULL	Ynr002cp	NucleicAcid		is a type of 					ATO protein	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_103_30_11142_s_57	16847258	Ynr002cp belongs to a family of ATO (ammonia/ammonium transport outward) proteins ( ) of which only three were represented in our data set and was not studied further.	gene_phenotype
70138	2	333645	11	NULL	NULL	0	NULL	ATO	GP		is					ammonia/ammonium transport outward	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_103_30_11142_s_57	16847258	Ynr002cp belongs to a family of ATO (ammonia/ammonium transport outward) proteins ( ) of which only three were represented in our data set and was not studied further.	gene_phenotype
70139	1	333646	11	NULL	NULL	NULL	NULL	 ATO3	GP		is a type of 					putative ammonia exporter	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_46_45882_s_191	12966084	What is the relationship between the elevated expression of  ATO3 (and other putative ammonia exporters,  YCR010c and  YNR002c; see Epstein  et al., Ref.  ) in respiratory deficient rhoo petite cells and ammonia production in respiratory competent cells in colonies that are in late stages of growth?	gene_phenotype
70140	2	333646	11	NULL	NULL	0	NULL	YCR010c	NucleicAcid		is a type of 					putative ammonia exporter	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_45882_s_191	12966084	What is the relationship between the elevated expression of  ATO3 (and other putative ammonia exporters,  YCR010c and  YNR002c; see Epstein  et al., Ref.  ) in respiratory deficient rhoo petite cells and ammonia production in respiratory competent cells in colonies that are in late stages of growth?	gene_phenotype
70141	3	333646	11	NULL	NULL	0	NULL	 YNR002c	NucleicAcid		is a type of 					putative ammonia exporter	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_46_45882_s_191	12966084	What is the relationship between the elevated expression of  ATO3 (and other putative ammonia exporters,  YCR010c and  YNR002c; see Epstein  et al., Ref.  ) in respiratory deficient rhoo petite cells and ammonia production in respiratory competent cells in colonies that are in late stages of growth?	gene_phenotype
71853	1	333647	11	NULL	NULL	0	NULL	Ddi1	GP		is a type of					ubiquitin like protein	GP				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_293_3_986_s_83	12051757	Since the search for a budding yeast database revealed the presence of two ubiquitin-like proteins, Ddi1 and Yol111c, we examined whether the two ubiquitin-like proteins Ddi1 and Yol111c, as well as Rad23 [ 11,  12,  13 and  14] and Dsk2 [ 12 and  15], can interact with polyubiquitinated proteins and also with the 26S proteasome.	gene_phenotype
71854	2	333647	11	NULL	NULL	0	NULL	Yol111c	NucleicAcid		is a type of 					ubiquitin like protein	GP				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_293_3_986_s_83	12051757	Since the search for a budding yeast database revealed the presence of two ubiquitin-like proteins, Ddi1 and Yol111c, we examined whether the two ubiquitin-like proteins Ddi1 and Yol111c, as well as Rad23 [ 11,  12,  13 and  14] and Dsk2 [ 12 and  15], can interact with polyubiquitinated proteins and also with the 26S proteasome.	gene_phenotype
71855	3	333647	11	NULL	NULL	0	NULL	Ddi1	GP		interacts with		possibly			polyubiquitinated proteins	GP				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_293_3_986_s_83	12051757	Since the search for a budding yeast database revealed the presence of two ubiquitin-like proteins, Ddi1 and Yol111c, we examined whether the two ubiquitin-like proteins Ddi1 and Yol111c, as well as Rad23 [ 11,  12,  13 and  14] and Dsk2 [ 12 and  15], can interact with polyubiquitinated proteins and also with the 26S proteasome.	gene_phenotype
71856	4	333647	11	NULL	NULL	0	NULL	Ddi1	GP		interacts with 		possibly			26S proteasome	Cell Component				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_293_3_986_s_83	12051757	Since the search for a budding yeast database revealed the presence of two ubiquitin-like proteins, Ddi1 and Yol111c, we examined whether the two ubiquitin-like proteins Ddi1 and Yol111c, as well as Rad23 [ 11,  12,  13 and  14] and Dsk2 [ 12 and  15], can interact with polyubiquitinated proteins and also with the 26S proteasome.	gene_phenotype
71857	5	333647	11	NULL	NULL	0	NULL	Yol111c	NucleicAcid		interacts with		possibly			polyubiquitinated proteins	GP				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_293_3_986_s_83	12051757	Since the search for a budding yeast database revealed the presence of two ubiquitin-like proteins, Ddi1 and Yol111c, we examined whether the two ubiquitin-like proteins Ddi1 and Yol111c, as well as Rad23 [ 11,  12,  13 and  14] and Dsk2 [ 12 and  15], can interact with polyubiquitinated proteins and also with the 26S proteasome.	gene_phenotype
71858	6	333647	11	NULL	NULL	0	NULL	Yol111c	NucleicAcid		interacts with 		possibly			26S proteasome	Cell Component				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_293_3_986_s_83	12051757	Since the search for a budding yeast database revealed the presence of two ubiquitin-like proteins, Ddi1 and Yol111c, we examined whether the two ubiquitin-like proteins Ddi1 and Yol111c, as well as Rad23 [ 11,  12,  13 and  14] and Dsk2 [ 12 and  15], can interact with polyubiquitinated proteins and also with the 26S proteasome.	gene_phenotype
71859	7	333647	11	NULL	NULL	0	NULL	 Rad 23	GP		interacts with		possibly			polyubiquitinated proteins	GP				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_293_3_986_s_83	12051757	Since the search for a budding yeast database revealed the presence of two ubiquitin-like proteins, Ddi1 and Yol111c, we examined whether the two ubiquitin-like proteins Ddi1 and Yol111c, as well as Rad23 [ 11,  12,  13 and  14] and Dsk2 [ 12 and  15], can interact with polyubiquitinated proteins and also with the 26S proteasome.	gene_phenotype
71860	8	333647	11	NULL	NULL	NULL	NULL	Rad 23	GP		interacts with		possibly			26S proteasome	Cell Component				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_293_3_986_s_83	12051757	Since the search for a budding yeast database revealed the presence of two ubiquitin-like proteins, Ddi1 and Yol111c, we examined whether the two ubiquitin-like proteins Ddi1 and Yol111c, as well as Rad23 [ 11,  12,  13 and  14] and Dsk2 [ 12 and  15], can interact with polyubiquitinated proteins and also with the 26S proteasome.	gene_phenotype
71861	9	333647	11	NULL	NULL	0	NULL	Dsk2	GP		interacts with 		possibly			polyubiquitinated proteins	GP				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_293_3_986_s_83	12051757	Since the search for a budding yeast database revealed the presence of two ubiquitin-like proteins, Ddi1 and Yol111c, we examined whether the two ubiquitin-like proteins Ddi1 and Yol111c, as well as Rad23 [ 11,  12,  13 and  14] and Dsk2 [ 12 and  15], can interact with polyubiquitinated proteins and also with the 26S proteasome.	gene_phenotype
71862	10	333647	11	NULL	NULL	0	NULL	Dsk2	GP		interacts with 		possibly			26S proteasome	Cell Component				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_293_3_986_s_83	12051757	Since the search for a budding yeast database revealed the presence of two ubiquitin-like proteins, Ddi1 and Yol111c, we examined whether the two ubiquitin-like proteins Ddi1 and Yol111c, as well as Rad23 [ 11,  12,  13 and  14] and Dsk2 [ 12 and  15], can interact with polyubiquitinated proteins and also with the 26S proteasome.	gene_phenotype
70142	1	333650	11	NULL	NULL	0	NULL	 YAL048c protein	NucleicAcid		 is involved in					vesicle transport	Process	 in the secretory pathway			NULL		0	NULL	NULL	NULL	abs-batch0680-0699_yeast_15_5_10220001_s_10	10220001	We suggest that the YAL048c protein is involved in vesicle transport  in the secretory pathway.	gene_phenotype
70143	1	333651	11	NULL	NULL	0	NULL	 Sso1 	GP		is a type of 					syntaxin	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_1_s_224	12489121	Overexpression of syntaxins Sso1 and Sso2, functioning  at the targeting/fusion of the Golgi-derived secretory vesicles to the plasma membrane,  polyubiquitin,  PSE1 and YAL048c ORF or the disruption of protease Yps1p, Yap3p encoding genes also enhance  heterologous protein secretion (Knittler and Haas, [ 1992]; Chow  et al., [ 1992]; Chen  et al., [ 1994]; Robinson  et al., [ 1994]; Ruohonen  et al., [ 1997];	gene_phenotype
70144	2	333651	11	NULL	NULL	0	NULL	Sso2	GP		is a type of 					syntaxin	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_1_s_224	12489121	Overexpression of syntaxins Sso1 and Sso2, functioning  at the targeting/fusion of the Golgi-derived secretory vesicles to the plasma membrane,  polyubiquitin,  PSE1 and YAL048c ORF or the disruption of protease Yps1p, Yap3p encoding genes also enhance  heterologous protein secretion (Knittler and Haas, [ 1992]; Chow  et al., [ 1992]; Chen  et al., [ 1994]; Robinson  et al., [ 1994]; Ruohonen  et al., [ 1997];	gene_phenotype
70483	3	333651	11	NULL	NULL	0	NULL	secretory vesicles	cell component		is derived from					Golgi	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_1_s_224	12489121	Overexpression of syntaxins Sso1 and Sso2, functioning  at the targeting/fusion of the Golgi-derived secretory vesicles to the plasma membrane,  polyubiquitin,  PSE1 and YAL048c ORF or the disruption of protease Yps1p, Yap3p encoding genes also enhance  heterologous protein secretion (Knittler and Haas, [ 1992]; Chow  et al., [ 1992]; Chen  et al., [ 1994]; Robinson  et al., [ 1994]; Ruohonen  et al., [ 1997];	gene_phenotype
70484	4	333651	11	NULL	NULL	0	NULL	statement 3	cell component		is targeted to					 plasma membrane	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_1_s_224	12489121	Overexpression of syntaxins Sso1 and Sso2, functioning  at the targeting/fusion of the Golgi-derived secretory vesicles to the plasma membrane,  polyubiquitin,  PSE1 and YAL048c ORF or the disruption of protease Yps1p, Yap3p encoding genes also enhance  heterologous protein secretion (Knittler and Haas, [ 1992]; Chow  et al., [ 1992]; Chen  et al., [ 1994]; Robinson  et al., [ 1994]; Ruohonen  et al., [ 1997];	gene_phenotype
70485	5	333651	11	NULL	NULL	0	NULL	statement 3	cell component		is fused to 					 plasma membrane	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_1_s_224	12489121	Overexpression of syntaxins Sso1 and Sso2, functioning  at the targeting/fusion of the Golgi-derived secretory vesicles to the plasma membrane,  polyubiquitin,  PSE1 and YAL048c ORF or the disruption of protease Yps1p, Yap3p encoding genes also enhance  heterologous protein secretion (Knittler and Haas, [ 1992]; Chow  et al., [ 1992]; Chen  et al., [ 1994]; Robinson  et al., [ 1994]; Ruohonen  et al., [ 1997];	gene_phenotype
70486	6	333651	11	NULL	NULL	0	NULL	statement 4	Process		ia alternative to 					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_1_s_224	12489121	Overexpression of syntaxins Sso1 and Sso2, functioning  at the targeting/fusion of the Golgi-derived secretory vesicles to the plasma membrane,  polyubiquitin,  PSE1 and YAL048c ORF or the disruption of protease Yps1p, Yap3p encoding genes also enhance  heterologous protein secretion (Knittler and Haas, [ 1992]; Chow  et al., [ 1992]; Chen  et al., [ 1994]; Robinson  et al., [ 1994]; Ruohonen  et al., [ 1997];	gene_phenotype
70487	7	333651	11	NULL	NULL	0	NULL	Sso1	GP		plays a role in					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_1_s_224	12489121	Overexpression of syntaxins Sso1 and Sso2, functioning  at the targeting/fusion of the Golgi-derived secretory vesicles to the plasma membrane,  polyubiquitin,  PSE1 and YAL048c ORF or the disruption of protease Yps1p, Yap3p encoding genes also enhance  heterologous protein secretion (Knittler and Haas, [ 1992]; Chow  et al., [ 1992]; Chen  et al., [ 1994]; Robinson  et al., [ 1994]; Ruohonen  et al., [ 1997];	gene_phenotype
70488	8	333651	11	NULL	NULL	0	NULL	Sso1	GP		plays a role in					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_1_s_224	12489121	Overexpression of syntaxins Sso1 and Sso2, functioning  at the targeting/fusion of the Golgi-derived secretory vesicles to the plasma membrane,  polyubiquitin,  PSE1 and YAL048c ORF or the disruption of protease Yps1p, Yap3p encoding genes also enhance  heterologous protein secretion (Knittler and Haas, [ 1992]; Chow  et al., [ 1992]; Chen  et al., [ 1994]; Robinson  et al., [ 1994]; Ruohonen  et al., [ 1997];	gene_phenotype
70489	9	333651	11	NULL	NULL	0	NULL	Sso1	GP	Overexpression of	enhance					protein	GP	secretion of;;heterologous			NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_1_s_224	12489121	Overexpression of syntaxins Sso1 and Sso2, functioning  at the targeting/fusion of the Golgi-derived secretory vesicles to the plasma membrane,  polyubiquitin,  PSE1 and YAL048c ORF or the disruption of protease Yps1p, Yap3p encoding genes also enhance  heterologous protein secretion (Knittler and Haas, [ 1992]; Chow  et al., [ 1992]; Chen  et al., [ 1994]; Robinson  et al., [ 1994]; Ruohonen  et al., [ 1997];	gene_phenotype
70501	10	333651	11	NULL	NULL	0	NULL	Sso2	GP		plays a role in					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_1_s_224	12489121	Overexpression of syntaxins Sso1 and Sso2, functioning  at the targeting/fusion of the Golgi-derived secretory vesicles to the plasma membrane,  polyubiquitin,  PSE1 and YAL048c ORF or the disruption of protease Yps1p, Yap3p encoding genes also enhance  heterologous protein secretion (Knittler and Haas, [ 1992]; Chow  et al., [ 1992]; Chen  et al., [ 1994]; Robinson  et al., [ 1994]; Ruohonen  et al., [ 1997];	gene_phenotype
70502	11	333651	11	NULL	NULL	0	NULL	Sso2	GP		plays a role in					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_1_s_224	12489121	Overexpression of syntaxins Sso1 and Sso2, functioning  at the targeting/fusion of the Golgi-derived secretory vesicles to the plasma membrane,  polyubiquitin,  PSE1 and YAL048c ORF or the disruption of protease Yps1p, Yap3p encoding genes also enhance  heterologous protein secretion (Knittler and Haas, [ 1992]; Chow  et al., [ 1992]; Chen  et al., [ 1994]; Robinson  et al., [ 1994]; Ruohonen  et al., [ 1997];	gene_phenotype
70503	12	333651	11	10	NULL	NULL	NULL	Sso2	GP	overexpression of	enhance					protein	GP	secretion of;;heterologous			NULL		NULL	NULL	NULL	NULL	gw70_yeast_20_1_1_s_224	12489121	Overexpression of syntaxins Sso1 and Sso2, functioning  at the targeting/fusion of the Golgi-derived secretory vesicles to the plasma membrane,  polyubiquitin,  PSE1 and YAL048c ORF or the disruption of protease Yps1p, Yap3p encoding genes also enhance  heterologous protein secretion (Knittler and Haas, [ 1992]; Chow  et al., [ 1992]; Chen  et al., [ 1994]; Robinson  et al., [ 1994]; Ruohonen  et al., [ 1997];	gene_phenotype
70504	13	333651	11	NULL	NULL	0	NULL	polyubiquitin	GP		enhance					protein	GP	secretion of;;heterologous			NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_1_s_224	12489121	Overexpression of syntaxins Sso1 and Sso2, functioning  at the targeting/fusion of the Golgi-derived secretory vesicles to the plasma membrane,  polyubiquitin,  PSE1 and YAL048c ORF or the disruption of protease Yps1p, Yap3p encoding genes also enhance  heterologous protein secretion (Knittler and Haas, [ 1992]; Chow  et al., [ 1992]; Chen  et al., [ 1994]; Robinson  et al., [ 1994]; Ruohonen  et al., [ 1997];	gene_phenotype
70505	14	333651	11	NULL	NULL	0	NULL	PSE1	GP		enhance					protein	GP	secretion of;;heterologous			NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_1_s_224	12489121	Overexpression of syntaxins Sso1 and Sso2, functioning  at the targeting/fusion of the Golgi-derived secretory vesicles to the plasma membrane,  polyubiquitin,  PSE1 and YAL048c ORF or the disruption of protease Yps1p, Yap3p encoding genes also enhance  heterologous protein secretion (Knittler and Haas, [ 1992]; Chow  et al., [ 1992]; Chen  et al., [ 1994]; Robinson  et al., [ 1994]; Ruohonen  et al., [ 1997];	gene_phenotype
70506	15	333651	11	NULL	NULL	0	NULL	YAL048c ORF	NucleicAcid		enhance					protein	GP	secretion of;;heterologous			NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_1_s_224	12489121	Overexpression of syntaxins Sso1 and Sso2, functioning  at the targeting/fusion of the Golgi-derived secretory vesicles to the plasma membrane,  polyubiquitin,  PSE1 and YAL048c ORF or the disruption of protease Yps1p, Yap3p encoding genes also enhance  heterologous protein secretion (Knittler and Haas, [ 1992]; Chow  et al., [ 1992]; Chen  et al., [ 1994]; Robinson  et al., [ 1994]; Ruohonen  et al., [ 1997];	gene_phenotype
70507	16	333651	11	NULL	NULL	0	NULL	Yps1p gene	GP	disruption of	enhance					protein	GP	secretion of;;heterologous			NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_1_s_224	12489121	Overexpression of syntaxins Sso1 and Sso2, functioning  at the targeting/fusion of the Golgi-derived secretory vesicles to the plasma membrane,  polyubiquitin,  PSE1 and YAL048c ORF or the disruption of protease Yps1p, Yap3p encoding genes also enhance  heterologous protein secretion (Knittler and Haas, [ 1992]; Chow  et al., [ 1992]; Chen  et al., [ 1994]; Robinson  et al., [ 1994]; Ruohonen  et al., [ 1997];	gene_phenotype
70508	17	333651	11	NULL	NULL	0	NULL	Yap3p gene	GP	disruption of	enhance					protein	GP	secretion of;;heterologous			NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_1_s_224	12489121	Overexpression of syntaxins Sso1 and Sso2, functioning  at the targeting/fusion of the Golgi-derived secretory vesicles to the plasma membrane,  polyubiquitin,  PSE1 and YAL048c ORF or the disruption of protease Yps1p, Yap3p encoding genes also enhance  heterologous protein secretion (Knittler and Haas, [ 1992]; Chow  et al., [ 1992]; Chen  et al., [ 1994]; Robinson  et al., [ 1994]; Ruohonen  et al., [ 1997];	gene_phenotype
71863	18	333651	11	NULL	NULL	0	NULL	Yps1p	GP		is a type of 					protease	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_1_s_224	12489121	Overexpression of syntaxins Sso1 and Sso2, functioning  at the targeting/fusion of the Golgi-derived secretory vesicles to the plasma membrane,  polyubiquitin,  PSE1 and YAL048c ORF or the disruption of protease Yps1p, Yap3p encoding genes also enhance  heterologous protein secretion (Knittler and Haas, [ 1992]; Chow  et al., [ 1992]; Chen  et al., [ 1994]; Robinson  et al., [ 1994]; Ruohonen  et al., [ 1997];	gene_phenotype
71864	19	333651	11	NULL	NULL	0	NULL	Yps3p	GP		is a type of 					protease	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_1_s_224	12489121	Overexpression of syntaxins Sso1 and Sso2, functioning  at the targeting/fusion of the Golgi-derived secretory vesicles to the plasma membrane,  polyubiquitin,  PSE1 and YAL048c ORF or the disruption of protease Yps1p, Yap3p encoding genes also enhance  heterologous protein secretion (Knittler and Haas, [ 1992]; Chow  et al., [ 1992]; Chen  et al., [ 1994]; Robinson  et al., [ 1994]; Ruohonen  et al., [ 1997];	gene_phenotype
70145	1	333654	11	NULL	NULL	0	NULL	YDL193w	NucleicAcid	Null mutations	is					 lethal	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_485_1_29_s_112	11086160	Null mutations of YDL193w are lethal, thus, the gene was a suitable test system for the N-terminal tagging method since malfunction of the Cre/lox system or frame-shift mutations caused by mis-integration of yEGFP would result in loss of function and therefore loss of viability.	gene_phenotype
70152	1	333658	11	NULL	NULL	NULL	NULL	YOR1 gene	GP	S. cerevisiae homolog	transports					 small molecule 	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803598_s_10	16803598	Homologues of 10 S. cerevisiae  genes previously shown to be Pdr1-Pdr3 targets were upregulated (YOR1,  RTA1, RSB1, RPN4, YLR346c and YMR102c along with CDR1, PDH1 and PDR1 itself)  or downregulated (PDR12); roles for these genes include small molecule  transport and transcriptional regulation.	gene_phenotype
70154	2	333658	11	NULL	NULL	NULL	NULL	RTA1 gene	GP	S. cerevisiae homolog	transports					 small molecule 	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803598_s_10	16803598	Homologues of 10 S. cerevisiae  genes previously shown to be Pdr1-Pdr3 targets were upregulated (YOR1,  RTA1, RSB1, RPN4, YLR346c and YMR102c along with CDR1, PDH1 and PDR1 itself)  or downregulated (PDR12); roles for these genes include small molecule  transport and transcriptional regulation.	gene_phenotype
70155	3	333658	11	NULL	NULL	NULL	NULL	RSB1 gene	GP	S. cerevisiae homolog	transports					 small molecule 	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803598_s_10	16803598	Homologues of 10 S. cerevisiae  genes previously shown to be Pdr1-Pdr3 targets were upregulated (YOR1,  RTA1, RSB1, RPN4, YLR346c and YMR102c along with CDR1, PDH1 and PDR1 itself)  or downregulated (PDR12); roles for these genes include small molecule  transport and transcriptional regulation.	gene_phenotype
70509	4	333658	11	NULL	NULL	NULL	NULL	RPN4 gene	GP	S. cerevisiae homolog	transports					small molecule	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803598_s_10	16803598	Homologues of 10 S. cerevisiae  genes previously shown to be Pdr1-Pdr3 targets were upregulated (YOR1,  RTA1, RSB1, RPN4, YLR346c and YMR102c along with CDR1, PDH1 and PDR1 itself)  or downregulated (PDR12); roles for these genes include small molecule  transport and transcriptional regulation.	gene_phenotype
70510	5	333658	11	NULL	NULL	0	NULL	YLR346c gene	GP	S. cerevisiae homolog	transports					small molecule	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803598_s_10	16803598	Homologues of 10 S. cerevisiae  genes previously shown to be Pdr1-Pdr3 targets were upregulated (YOR1,  RTA1, RSB1, RPN4, YLR346c and YMR102c along with CDR1, PDH1 and PDR1 itself)  or downregulated (PDR12); roles for these genes include small molecule  transport and transcriptional regulation.	gene_phenotype
70511	6	333658	11	NULL	NULL	0	NULL	YMR102c gene	GP	S. cerevisiae homolog	transports					small molecule	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803598_s_10	16803598	Homologues of 10 S. cerevisiae  genes previously shown to be Pdr1-Pdr3 targets were upregulated (YOR1,  RTA1, RSB1, RPN4, YLR346c and YMR102c along with CDR1, PDH1 and PDR1 itself)  or downregulated (PDR12); roles for these genes include small molecule  transport and transcriptional regulation.	gene_phenotype
70512	7	333658	11	NULL	NULL	0	NULL	CDR1 gene	GP	S. cerevisiae homolog	transports					small molecule	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803598_s_10	16803598	Homologues of 10 S. cerevisiae  genes previously shown to be Pdr1-Pdr3 targets were upregulated (YOR1,  RTA1, RSB1, RPN4, YLR346c and YMR102c along with CDR1, PDH1 and PDR1 itself)  or downregulated (PDR12); roles for these genes include small molecule  transport and transcriptional regulation.	gene_phenotype
70513	8	333658	11	NULL	NULL	0	NULL	PDH1 gene	GP	S. cerevisiae homolog	transports					small molecule	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803598_s_10	16803598	Homologues of 10 S. cerevisiae  genes previously shown to be Pdr1-Pdr3 targets were upregulated (YOR1,  RTA1, RSB1, RPN4, YLR346c and YMR102c along with CDR1, PDH1 and PDR1 itself)  or downregulated (PDR12); roles for these genes include small molecule  transport and transcriptional regulation.	gene_phenotype
70514	9	333658	11	NULL	NULL	0	NULL	PDR1  gene	GP	S. cerevisiae homolog	transports					small molecule	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803598_s_10	16803598	Homologues of 10 S. cerevisiae  genes previously shown to be Pdr1-Pdr3 targets were upregulated (YOR1,  RTA1, RSB1, RPN4, YLR346c and YMR102c along with CDR1, PDH1 and PDR1 itself)  or downregulated (PDR12); roles for these genes include small molecule  transport and transcriptional regulation.	gene_phenotype
70515	10	333658	11	NULL	NULL	0	NULL	PDR12 gene	GP	S. cerevisiae homolog	transports					small molecule	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803598_s_10	16803598	Homologues of 10 S. cerevisiae  genes previously shown to be Pdr1-Pdr3 targets were upregulated (YOR1,  RTA1, RSB1, RPN4, YLR346c and YMR102c along with CDR1, PDH1 and PDR1 itself)  or downregulated (PDR12); roles for these genes include small molecule  transport and transcriptional regulation.	gene_phenotype
70516	11	333658	11	NULL	NULL	0	NULL	YOR1 gene	GP	S. cerevisiae homolog	regulate					transcription 	Process				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803598_s_10	16803598	Homologues of 10 S. cerevisiae  genes previously shown to be Pdr1-Pdr3 targets were upregulated (YOR1,  RTA1, RSB1, RPN4, YLR346c and YMR102c along with CDR1, PDH1 and PDR1 itself)  or downregulated (PDR12); roles for these genes include small molecule  transport and transcriptional regulation.	gene_phenotype
70517	12	333658	11	NULL	NULL	0	NULL	RTA1 gene	GP	S. cerevisiae homolog	regulate					transcription	Process				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803598_s_10	16803598	Homologues of 10 S. cerevisiae  genes previously shown to be Pdr1-Pdr3 targets were upregulated (YOR1,  RTA1, RSB1, RPN4, YLR346c and YMR102c along with CDR1, PDH1 and PDR1 itself)  or downregulated (PDR12); roles for these genes include small molecule  transport and transcriptional regulation.	gene_phenotype
70518	13	333658	11	NULL	NULL	0	NULL	RSB1 gene	GP	S. cerevisiae homolog	regulate					transcription	Process				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803598_s_10	16803598	Homologues of 10 S. cerevisiae  genes previously shown to be Pdr1-Pdr3 targets were upregulated (YOR1,  RTA1, RSB1, RPN4, YLR346c and YMR102c along with CDR1, PDH1 and PDR1 itself)  or downregulated (PDR12); roles for these genes include small molecule  transport and transcriptional regulation.	gene_phenotype
70519	14	333658	11	NULL	NULL	0	NULL	RPN4 gene	GP	S. cerevisiae homolog	regulate					transcription	Process				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803598_s_10	16803598	Homologues of 10 S. cerevisiae  genes previously shown to be Pdr1-Pdr3 targets were upregulated (YOR1,  RTA1, RSB1, RPN4, YLR346c and YMR102c along with CDR1, PDH1 and PDR1 itself)  or downregulated (PDR12); roles for these genes include small molecule  transport and transcriptional regulation.	gene_phenotype
70520	15	333658	11	NULL	NULL	0	NULL	YLR346c gene	GP	S. cerevisiae homolog	regulate					transcription	Process				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803598_s_10	16803598	Homologues of 10 S. cerevisiae  genes previously shown to be Pdr1-Pdr3 targets were upregulated (YOR1,  RTA1, RSB1, RPN4, YLR346c and YMR102c along with CDR1, PDH1 and PDR1 itself)  or downregulated (PDR12); roles for these genes include small molecule  transport and transcriptional regulation.	gene_phenotype
70521	16	333658	11	NULL	NULL	0	NULL	YMR102c gene	GP	S. cerevisiae homolog	regulate					transcription	Process				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803598_s_10	16803598	Homologues of 10 S. cerevisiae  genes previously shown to be Pdr1-Pdr3 targets were upregulated (YOR1,  RTA1, RSB1, RPN4, YLR346c and YMR102c along with CDR1, PDH1 and PDR1 itself)  or downregulated (PDR12); roles for these genes include small molecule  transport and transcriptional regulation.	gene_phenotype
70522	17	333658	11	NULL	NULL	0	NULL	CDR1 gene	GP	S. cerevisiae homolog	regulate					transcription	Process				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803598_s_10	16803598	Homologues of 10 S. cerevisiae  genes previously shown to be Pdr1-Pdr3 targets were upregulated (YOR1,  RTA1, RSB1, RPN4, YLR346c and YMR102c along with CDR1, PDH1 and PDR1 itself)  or downregulated (PDR12); roles for these genes include small molecule  transport and transcriptional regulation.	gene_phenotype
70523	18	333658	11	NULL	NULL	0	NULL	PDH1 gene	GP	S. cerevisiae homolog	regulate					transcription	Process				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803598_s_10	16803598	Homologues of 10 S. cerevisiae  genes previously shown to be Pdr1-Pdr3 targets were upregulated (YOR1,  RTA1, RSB1, RPN4, YLR346c and YMR102c along with CDR1, PDH1 and PDR1 itself)  or downregulated (PDR12); roles for these genes include small molecule  transport and transcriptional regulation.	gene_phenotype
70524	19	333658	11	NULL	NULL	0	NULL	PDR1  gene	GP	S. cerevisiae homolog	regulate					transcription	Process				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803598_s_10	16803598	Homologues of 10 S. cerevisiae  genes previously shown to be Pdr1-Pdr3 targets were upregulated (YOR1,  RTA1, RSB1, RPN4, YLR346c and YMR102c along with CDR1, PDH1 and PDR1 itself)  or downregulated (PDR12); roles for these genes include small molecule  transport and transcriptional regulation.	gene_phenotype
70525	20	333658	11	NULL	NULL	0	NULL	PDR12 gene	GP	S. cerevisiae homolog	regulate					transcription	Process				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_mol-microbiol_61_3_16803598_s_10	16803598	Homologues of 10 S. cerevisiae  genes previously shown to be Pdr1-Pdr3 targets were upregulated (YOR1,  RTA1, RSB1, RPN4, YLR346c and YMR102c along with CDR1, PDH1 and PDR1 itself)  or downregulated (PDR12); roles for these genes include small molecule  transport and transcriptional regulation.	gene_phenotype
70291	1	333660	11	NULL	NULL	0	NULL	 gamma-ray	Chemical		induced					mitotic interchromosomal recombination	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_mutat-res_486_1_11356335_s_6	11356335	REC41 is required for normal  levels of interplasmid recombination and gamma-ray induced mitotic interchromosomal  recombination.	gene_phenotype
70292	2	333660	11	NULL	NULL	0	NULL	REC41	GP		is required for 					statement 1	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_mutat-res_486_1_11356335_s_6	11356335	REC41 is required for normal  levels of interplasmid recombination and gamma-ray induced mitotic interchromosomal  recombination.	gene_phenotype
70293	3	333660	11	NULL	NULL	0	NULL	REC41	GP		is required for 					 interplasmid recombination	Process	normal level			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_mutat-res_486_1_11356335_s_6	11356335	REC41 is required for normal  levels of interplasmid recombination and gamma-ray induced mitotic interchromosomal  recombination.	gene_phenotype
70294	1	333661	11	NULL	NULL	0	NULL	rec41	GP		undergoes					mutation	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_mutat-res_486_1_11356335_s_13	11356335	The rec41 mutation has an effect  on meiosis, likely meiotic recombination, even in the heterozygous state.	gene_phenotype
70295	2	333661	11	NULL	NULL	0	NULL	statement 1	Process		has an effect on					meiosis	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_mutat-res_486_1_11356335_s_13	11356335	The rec41 mutation has an effect  on meiosis, likely meiotic recombination, even in the heterozygous state.	gene_phenotype
70296	3	333661	11	NULL	NULL	0	NULL	statement 1	Process		has an effect on					meiotic recombination	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_mutat-res_486_1_11356335_s_13	11356335	The rec41 mutation has an effect  on meiosis, likely meiotic recombination, even in the heterozygous state.	gene_phenotype
70297	4	333661	11	NULL	NULL	0	NULL	statement 1	Process		has an effect on					heterozygous state	Chromosome				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_mutat-res_486_1_11356335_s_13	11356335	The rec41 mutation has an effect  on meiosis, likely meiotic recombination, even in the heterozygous state.	gene_phenotype
70298	1	333662	11	NULL	NULL	0	NULL	REC46 gene	GP	Saccharomyes cerevisiae	controls					mitotic chromosomal stablity	Chromosome				NULL		0	NULL	NULL	NULL	gw70_yeast_19_6_553_s_370	11921104	The  REC46 gene of  Saccharomyes cerevisiae controls mitotic chromosomal stablity, recombination and sporulation: cell-type and  life cycle stage-specific expression of  rec46-1 mutation.	gene_phenotype
70299	2	333662	11	NULL	NULL	0	NULL	REC46 gene	GP	Saccharomyes cerevisiae	controls					recombination	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_19_6_553_s_370	11921104	The  REC46 gene of  Saccharomyes cerevisiae controls mitotic chromosomal stablity, recombination and sporulation: cell-type and  life cycle stage-specific expression of  rec46-1 mutation.	gene_phenotype
70300	3	333662	11	NULL	NULL	0	NULL	REC46 gene	GP	Saccharomyes cerevisiae	controls					sporulation	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_19_6_553_s_370	11921104	The  REC46 gene of  Saccharomyes cerevisiae controls mitotic chromosomal stablity, recombination and sporulation: cell-type and  life cycle stage-specific expression of  rec46-1 mutation.	gene_phenotype
70301	1	333664	11	NULL	NULL	0	NULL	YLR324w gene	GP	deletion	alter					peroxisome	CellComponent	number;;size			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_2_665_s_178	14617799	Cells harboring deletions in one or more of the  YLR324w, YGR004w and  YBR168w genes exhibit peroxisomes that are altered in number and/or size.	gene_phenotype
70302	2	333664	11	NULL	NULL	0	NULL	YGR004w  gene	GP	deletion	alter					peroxisome	CellComponent	number;;size			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_2_665_s_178	14617799	Cells harboring deletions in one or more of the  YLR324w, YGR004w and  YBR168w genes exhibit peroxisomes that are altered in number and/or size.	gene_phenotype
70303	3	333664	11	NULL	NULL	0	NULL	YBR168w gene	GP	deletion	alter					peroxisome	CellComponent	number;;size			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_2_665_s_178	14617799	Cells harboring deletions in one or more of the  YLR324w, YGR004w and  YBR168w genes exhibit peroxisomes that are altered in number and/or size.	gene_phenotype
70304	1	333666	11	NULL	NULL	0	NULL	YLR324w gene	GP	S. cerevisiae	controls					peroxisome	CellComponent	number;;size			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_2_665_s_281	14617799	Many proteins, including those encoded by the genes  YLR324w, YGR004w, and  YBR168w of  S. cerevisiae, are involved in controlling peroxisome number and size in the cell.	gene_phenotype
70305	2	333666	11	NULL	NULL	0	NULL	YGR004w  gene	GP	S. cerevisiae	controls					peroxisome	CellComponent	number;;size			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_2_665_s_281	14617799	Many proteins, including those encoded by the genes  YLR324w, YGR004w, and  YBR168w of  S. cerevisiae, are involved in controlling peroxisome number and size in the cell.	gene_phenotype
70306	3	333666	11	NULL	NULL	0	NULL	YBR168w gene	GP	S. cerevisiae	controls					peroxisome	CellComponent	number;;size			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_2_665_s_281	14617799	Many proteins, including those encoded by the genes  YLR324w, YGR004w, and  YBR168w of  S. cerevisiae, are involved in controlling peroxisome number and size in the cell.	gene_phenotype
70307	1	333667	11	NULL	NULL	NULL	NULL	YLR324w gene	GP	deletion	increased					peroxisome	CellComponent	number;;size;;clustering			NULL	 strain DK2 	NULL	NULL	NULL	NULL	gw70_molbiolcell_15_2_665_s_174	14617799	Cells of strain  DK2 ( Figure 5F) carrying deletions in the  YLR324w and  YBR168w genes showed increased numbers of peroxisomes ( Table 3) of normal to enlarged size ( Figure 5I), some of which exhibited clustering, whereas cells of strain  DK3 ( Figure 5G) deleted for the  YGR004w and  YBR168w genes also contained greatly enlarged peroxisomes ( Figure 5I;  Table 3).	gene_phenotype
70308	2	333667	11	NULL	NULL	NULL	NULL	YBR168w gene	GP	deletion	increased					peroxisome	CellComponent	number;;size;;clustering			NULL	 strain DK2 	NULL	NULL	NULL	NULL	gw70_molbiolcell_15_2_665_s_174	14617799	Cells of strain  DK2 ( Figure 5F) carrying deletions in the  YLR324w and  YBR168w genes showed increased numbers of peroxisomes ( Table 3) of normal to enlarged size ( Figure 5I), some of which exhibited clustering, whereas cells of strain  DK3 ( Figure 5G) deleted for the  YGR004w and  YBR168w genes also contained greatly enlarged peroxisomes ( Figure 5I;  Table 3).	gene_phenotype
70309	3	333667	11	NULL	NULL	0	NULL	YGR004w  gene	GP	deletion	enlarged					peroxisomes	CellComponent				NULL	 strain DK3	0	NULL	NULL	NULL	gw70_molbiolcell_15_2_665_s_174	14617799	Cells of strain  DK2 ( Figure 5F) carrying deletions in the  YLR324w and  YBR168w genes showed increased numbers of peroxisomes ( Table 3) of normal to enlarged size ( Figure 5I), some of which exhibited clustering, whereas cells of strain  DK3 ( Figure 5G) deleted for the  YGR004w and  YBR168w genes also contained greatly enlarged peroxisomes ( Figure 5I;  Table 3).	gene_phenotype
70310	4	333667	11	NULL	NULL	0	NULL	YBR168w gene	GP	deletion	enlarged					peroxisome	CellComponent				NULL	 strain DK3	0	NULL	NULL	NULL	gw70_molbiolcell_15_2_665_s_174	14617799	Cells of strain  DK2 ( Figure 5F) carrying deletions in the  YLR324w and  YBR168w genes showed increased numbers of peroxisomes ( Table 3) of normal to enlarged size ( Figure 5I), some of which exhibited clustering, whereas cells of strain  DK3 ( Figure 5G) deleted for the  YGR004w and  YBR168w genes also contained greatly enlarged peroxisomes ( Figure 5I;  Table 3).	gene_phenotype
71865	1	333668	11	NULL	NULL	0	NULL	YGR004w	NucleicAcid	over expression of	complement		partially			peroxisomal morphology	physical phenomenon	abnormal			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_2_665_s_192	14617799	Overexpression of YGR004w Can Partially Complement the Abnormal Peroxisomal Morphology  Observed in Cells Deleted for One or Both of YLR324w and YBR168w   ecause cells deleted for one or more of the  YLR324w, YGR004w, and  YBR168w genes are compromised in their regulation of peroxisome size and number, we investigated the effects of overexpression of these genes on the overall peroxisome phenotype in cells harboring various combinations of deletions of these genes.	gene_phenotype
71866	2	333668	11	NULL	NULL	0	NULL	cells	Cell		deleted with					YLR324w	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_2_665_s_192	14617799	Overexpression of YGR004w Can Partially Complement the Abnormal Peroxisomal Morphology  Observed in Cells Deleted for One or Both of YLR324w and YBR168w   ecause cells deleted for one or more of the  YLR324w, YGR004w, and  YBR168w genes are compromised in their regulation of peroxisome size and number, we investigated the effects of overexpression of these genes on the overall peroxisome phenotype in cells harboring various combinations of deletions of these genes.	gene_phenotype
71867	3	333668	11	NULL	NULL	0	NULL	cells	Cell		deleted with					YBR168w	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_2_665_s_192	14617799	Overexpression of YGR004w Can Partially Complement the Abnormal Peroxisomal Morphology  Observed in Cells Deleted for One or Both of YLR324w and YBR168w   ecause cells deleted for one or more of the  YLR324w, YGR004w, and  YBR168w genes are compromised in their regulation of peroxisome size and number, we investigated the effects of overexpression of these genes on the overall peroxisome phenotype in cells harboring various combinations of deletions of these genes.	gene_phenotype
71868	4	333668	11	NULL	NULL	0	NULL	statement 1	Process		is observed in					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_2_665_s_192	14617799	Overexpression of YGR004w Can Partially Complement the Abnormal Peroxisomal Morphology  Observed in Cells Deleted for One or Both of YLR324w and YBR168w   ecause cells deleted for one or more of the  YLR324w, YGR004w, and  YBR168w genes are compromised in their regulation of peroxisome size and number, we investigated the effects of overexpression of these genes on the overall peroxisome phenotype in cells harboring various combinations of deletions of these genes.	gene_phenotype
71869	5	333668	11	NULL	NULL	0	NULL	statement 1	Process		is observed in					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_2_665_s_192	14617799	Overexpression of YGR004w Can Partially Complement the Abnormal Peroxisomal Morphology  Observed in Cells Deleted for One or Both of YLR324w and YBR168w   ecause cells deleted for one or more of the  YLR324w, YGR004w, and  YBR168w genes are compromised in their regulation of peroxisome size and number, we investigated the effects of overexpression of these genes on the overall peroxisome phenotype in cells harboring various combinations of deletions of these genes.	gene_phenotype
70481	1	333670	11	NULL	NULL	0	NULL	YER064C gene	GP		is a type of 		potential			small molecule transporter	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1517_2_177_s_204	11342098	YER064C is a gene of unknown function but is predicted to be a small molecule transporter localized to an integral membrane [  38].	gene_phenotype
70482	2	333670	11	NULL	NULL	0	NULL	YER064C gene	NucleicAcid		is localized to		potentially			 integral membrane	CellComponent				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1517_2_177_s_204	11342098	YER064C is a gene of unknown function but is predicted to be a small molecule transporter localized to an integral membrane [  38].	gene_phenotype
70318	1	333671	11	NULL	NULL	0	NULL	Yer064Cp	GP		is a type of 					 nuclear protein	GP				NULL		0	NULL	NULL	NULL	gw70_genetics_174_1_191_s_30	16783004	Yer064Cp, a nuclear protein of unknown function, is important for the activation of some  ERG genes ( ENNEDY et al;  ERMANN et al).	gene_phenotype
70319	2	333671	11	NULL	NULL	0	NULL	Yer064Cp	GP		activates					ERG genes	GP				NULL		0	NULL	NULL	NULL	gw70_genetics_174_1_191_s_30	16783004	Yer064Cp, a nuclear protein of unknown function, is important for the activation of some  ERG genes ( ENNEDY et al;  ERMANN et al).	gene_phenotype
70320	1	333672	11	NULL	NULL	0	NULL	 sst2	GP	mutant	 increases					pheromone sensitivity	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_5_2_330_s_8	16467474	A number of mutants produced an increase ( sst2,  bar1,  asc1, and  ygl024w) or decrease ( cla4) in pheromone sensitivity or resulted in pheromone-independent signaling ( sst2,  pbs2,  gas1, and  ygl024w).	gene_phenotype
70321	2	333672	11	NULL	NULL	0	NULL	bar1	GP	mutant	increases					pheromone sensitivity	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_5_2_330_s_8	16467474	A number of mutants produced an increase ( sst2,  bar1,  asc1, and  ygl024w) or decrease ( cla4) in pheromone sensitivity or resulted in pheromone-independent signaling ( sst2,  pbs2,  gas1, and  ygl024w).	gene_phenotype
70322	3	333672	11	NULL	NULL	0	NULL	asc1	GP	mutant	increases					pheromone sensitivity	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_5_2_330_s_8	16467474	A number of mutants produced an increase ( sst2,  bar1,  asc1, and  ygl024w) or decrease ( cla4) in pheromone sensitivity or resulted in pheromone-independent signaling ( sst2,  pbs2,  gas1, and  ygl024w).	gene_phenotype
70323	4	333672	11	NULL	NULL	0	NULL	ygl024w	GP	mutant	increases					pheromone sensitivity	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_5_2_330_s_8	16467474	A number of mutants produced an increase ( sst2,  bar1,  asc1, and  ygl024w) or decrease ( cla4) in pheromone sensitivity or resulted in pheromone-independent signaling ( sst2,  pbs2,  gas1, and  ygl024w).	gene_phenotype
70324	5	333672	11	NULL	NULL	0	NULL	cla4	GP	mutant	decreases					pheromone sensitivity	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_5_2_330_s_8	16467474	A number of mutants produced an increase ( sst2,  bar1,  asc1, and  ygl024w) or decrease ( cla4) in pheromone sensitivity or resulted in pheromone-independent signaling ( sst2,  pbs2,  gas1, and  ygl024w).	gene_phenotype
70325	6	333672	11	NULL	NULL	0	NULL	sst2	GP	mutant	resulted in 					pheromone-independent signaling 	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_5_2_330_s_8	16467474	A number of mutants produced an increase ( sst2,  bar1,  asc1, and  ygl024w) or decrease ( cla4) in pheromone sensitivity or resulted in pheromone-independent signaling ( sst2,  pbs2,  gas1, and  ygl024w).	gene_phenotype
70326	7	333672	11	NULL	NULL	0	NULL	 pbs2	GP	mutant	resulted in 					pheromone-independent signaling 	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_5_2_330_s_8	16467474	A number of mutants produced an increase ( sst2,  bar1,  asc1, and  ygl024w) or decrease ( cla4) in pheromone sensitivity or resulted in pheromone-independent signaling ( sst2,  pbs2,  gas1, and  ygl024w).	gene_phenotype
70329	8	333672	11	NULL	NULL	0	NULL	gas1	GP	mutant	resulted in 					pheromone-independent signaling	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_5_2_330_s_8	16467474	A number of mutants produced an increase ( sst2,  bar1,  asc1, and  ygl024w) or decrease ( cla4) in pheromone sensitivity or resulted in pheromone-independent signaling ( sst2,  pbs2,  gas1, and  ygl024w).	gene_phenotype
70330	9	333672	11	NULL	NULL	0	NULL	ygl024w	GP	mutant	resulted in 					pheromone-independent signaling	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_5_2_330_s_8	16467474	A number of mutants produced an increase ( sst2,  bar1,  asc1, and  ygl024w) or decrease ( cla4) in pheromone sensitivity or resulted in pheromone-independent signaling ( sst2,  pbs2,  gas1, and  ygl024w).	gene_phenotype
70334	1	333674	11	NULL	NULL	0	NULL	YGL024W	NucleicAcid	Deletion	removes					Pgd1 protein	GP		N-terminal		NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_5_2_330_s_432	16467474	Deletion of  YGL024W removes the N-terminal portion of the Pgd1 protein and enhances signaling activity, while deletion of the entire  PGD1 gene removes both the N-terminal and C-terminal portions, and signaling is unaffected.	gene_phenotype
70336	2	333674	11	NULL	NULL	0	NULL	statement 1	Process		activates					signaling	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_5_2_330_s_432	16467474	Deletion of  YGL024W removes the N-terminal portion of the Pgd1 protein and enhances signaling activity, while deletion of the entire  PGD1 gene removes both the N-terminal and C-terminal portions, and signaling is unaffected.	gene_phenotype
70356	1	333677	11	NULL	NULL	0	NULL	 SRO77 gene	GP		involved in					endocytosis	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_10_4075_s_365	15870279	Finally, genes involved in endocytosis ( SRO77 and  AKR2) were also up-regulated, including several (e.g.,  IZH4,  CLC1,  AKR1,  RVS161,  AFR1, and YBR108W) that were induced much earlier in the time course.	gene_phenotype
70357	2	333677	11	NULL	NULL	0	NULL	AKR2 gene	GP		involved in					endocytosis	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_10_4075_s_365	15870279	Finally, genes involved in endocytosis ( SRO77 and  AKR2) were also up-regulated, including several (e.g.,  IZH4,  CLC1,  AKR1,  RVS161,  AFR1, and YBR108W) that were induced much earlier in the time course.	gene_phenotype
70359	1	333679	11	NULL	NULL	0	NULL	YLR424W gene	NucleicAcid	 S. cerevisiae	required for					viability	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_12_1_5_s_192	12887888	For example, YLR424W, a  S. cerevisiae gene of unknown function required for viability and containing a G-patch putative RNA binding motif, is a component of T1 and T3-6.	gene_phenotype
70360	2	333679	11	NULL	NULL	0	NULL	YLR424W gene	NucleicAcid	S. cerevisiae	containing					G-patch putative RNA binding motif	GP				NULL		0	NULL	NULL	NULL	gw60_molcell_12_1_5_s_192	12887888	For example, YLR424W, a  S. cerevisiae gene of unknown function required for viability and containing a G-patch putative RNA binding motif, is a component of T1 and T3-6.	gene_phenotype
70361	3	333679	11	NULL	NULL	0	NULL	YLR424W gene	NucleicAcid	S. cerevisiae	 is a component of					 T1	GP				NULL		0	NULL	NULL	NULL	gw60_molcell_12_1_5_s_192	12887888	For example, YLR424W, a  S. cerevisiae gene of unknown function required for viability and containing a G-patch putative RNA binding motif, is a component of T1 and T3-6.	gene_phenotype
70363	4	333679	11	NULL	NULL	0	NULL	YLR424W gene	NucleicAcid	S. cerevisiae	is a component of					T3-6	GP				NULL		0	NULL	NULL	NULL	gw60_molcell_12_1_5_s_192	12887888	For example, YLR424W, a  S. cerevisiae gene of unknown function required for viability and containing a G-patch putative RNA binding motif, is a component of T1 and T3-6.	gene_phenotype
70366	1	333680	11	NULL	NULL	NULL	NULL	 YLR324w gene	NucleicAcid	deletion	increases					 peroxisome	CellComponent	number;;size			NULL	strain DK1	NULL	NULL	NULL	NULL	gw70_molbiolcell_15_2_665_s_173	14617799	Cells of strain  DK1 ( Figure 5E) carrying deletions in the  YLR324w and  YGR004w genes exhibited a mixed phenotype of increased numbers of peroxisomes ( Table 3) of normal to enlarged size ( Figure 5I;  Table 3).	gene_phenotype
70367	2	333680	11	NULL	NULL	0	NULL	YGR004w gene	NucleicAcid	deletion	increases					peroxisomes	CellComponent	number;;size			NULL	strain DK1	0	NULL	NULL	NULL	gw70_molbiolcell_15_2_665_s_173	14617799	Cells of strain  DK1 ( Figure 5E) carrying deletions in the  YLR324w and  YGR004w genes exhibited a mixed phenotype of increased numbers of peroxisomes ( Table 3) of normal to enlarged size ( Figure 5I;  Table 3).	gene_phenotype
70395	1	333682	11	NULL	NULL	0	NULL	SMK1	GP		encodes for					MAP kinase	GP	 sporulation pathway			NULL		0	NULL	NULL	NULL	gw60_genetics_163_3_875_s_286	12663529	Mutants in  SMK1,  MPK1, and  YKL161c, which encode, respectively, the MAP kinase of the sporulation pathway, the cell integrity pathway, and a putative uncharacterized pathway, are not toxin hypersensitive.	gene_phenotype
70396	2	333682	11	NULL	NULL	0	NULL	MPK1	GP		encodes for					MAP kinase	GP	cell integrity pathway			NULL		0	NULL	NULL	NULL	gw60_genetics_163_3_875_s_286	12663529	Mutants in  SMK1,  MPK1, and  YKL161c, which encode, respectively, the MAP kinase of the sporulation pathway, the cell integrity pathway, and a putative uncharacterized pathway, are not toxin hypersensitive.	gene_phenotype
70397	3	333682	11	NULL	NULL	0	NULL	YKL161c	GP		encodes for					MAP kinase	GP	 putative uncharacterized pathway			NULL		0	NULL	NULL	NULL	gw60_genetics_163_3_875_s_286	12663529	Mutants in  SMK1,  MPK1, and  YKL161c, which encode, respectively, the MAP kinase of the sporulation pathway, the cell integrity pathway, and a putative uncharacterized pathway, are not toxin hypersensitive.	gene_phenotype
70398	4	333682	11	NULL	NULL	0	NULL	statement 1	Process		is not hypersensitive to					toxin	Chemical				NULL		0	NULL	NULL	NULL	gw60_genetics_163_3_875_s_286	12663529	Mutants in  SMK1,  MPK1, and  YKL161c, which encode, respectively, the MAP kinase of the sporulation pathway, the cell integrity pathway, and a putative uncharacterized pathway, are not toxin hypersensitive.	gene_phenotype
70399	5	333682	11	NULL	NULL	0	NULL	statement 2	Process		is not hypersensitive to					toxin	Chemical				NULL		0	NULL	NULL	NULL	gw60_genetics_163_3_875_s_286	12663529	Mutants in  SMK1,  MPK1, and  YKL161c, which encode, respectively, the MAP kinase of the sporulation pathway, the cell integrity pathway, and a putative uncharacterized pathway, are not toxin hypersensitive.	gene_phenotype
70400	6	333682	11	NULL	NULL	0	NULL	statement 3	Process		is not hypersensitive to					toxin	Chemical				NULL		0	NULL	NULL	NULL	gw60_genetics_163_3_875_s_286	12663529	Mutants in  SMK1,  MPK1, and  YKL161c, which encode, respectively, the MAP kinase of the sporulation pathway, the cell integrity pathway, and a putative uncharacterized pathway, are not toxin hypersensitive.	gene_phenotype
70401	1	333683	11	NULL	NULL	0	NULL	YLR205c	NucleicAcid		is a type of 					 heme oxygenase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_11_7762_s_216	11112771	In a frataxin-deficient strain mitochondrial free iron accumulates and cannot be extruded from mitochondria, so that Aft1p encounters a low iron signal and stimulates the transcription of genes encoding the plasma membrane iron and siderophore transporters, the heme oxygenase (YLR205c) and the vacuolar iron transporter ( FET5/ FTH1).	gene_phenotype
70402	2	333683	11	NULL	NULL	0	NULL	FET5/ FTH1	GP		is a type of 					vacuolar iron transporter	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_11_7762_s_216	11112771	In a frataxin-deficient strain mitochondrial free iron accumulates and cannot be extruded from mitochondria, so that Aft1p encounters a low iron signal and stimulates the transcription of genes encoding the plasma membrane iron and siderophore transporters, the heme oxygenase (YLR205c) and the vacuolar iron transporter ( FET5/ FTH1).	gene_phenotype
70403	3	333683	11	NULL	NULL	NULL	NULL	 Aft1p	GP		stimulates					 YLR205c	GP	transcription of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_11_7762_s_216	11112771	In a frataxin-deficient strain mitochondrial free iron accumulates and cannot be extruded from mitochondria, so that Aft1p encounters a low iron signal and stimulates the transcription of genes encoding the plasma membrane iron and siderophore transporters, the heme oxygenase (YLR205c) and the vacuolar iron transporter ( FET5/ FTH1).	gene_phenotype
70404	4	333683	11	NULL	NULL	NULL	NULL	 Aft1p	GP		stimulates					FET5/ FTH1	GP	transcription of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_11_7762_s_216	11112771	In a frataxin-deficient strain mitochondrial free iron accumulates and cannot be extruded from mitochondria, so that Aft1p encounters a low iron signal and stimulates the transcription of genes encoding the plasma membrane iron and siderophore transporters, the heme oxygenase (YLR205c) and the vacuolar iron transporter ( FET5/ FTH1).	gene_phenotype
71870	5	333683	11	NULL	NULL	0	NULL	free iron	Chemical	mitochondrial	accumulates in					frataxin-deficient strain	Organism				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_11_7762_s_216	11112771	In a frataxin-deficient strain mitochondrial free iron accumulates and cannot be extruded from mitochondria, so that Aft1p encounters a low iron signal and stimulates the transcription of genes encoding the plasma membrane iron and siderophore transporters, the heme oxygenase (YLR205c) and the vacuolar iron transporter ( FET5/ FTH1).	gene_phenotype
71871	6	333683	11	NULL	NULL	0	NULL	free iron	Chemical	mitochondrial	is not extruded from					mitochondria	Cell Component				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_11_7762_s_216	11112771	In a frataxin-deficient strain mitochondrial free iron accumulates and cannot be extruded from mitochondria, so that Aft1p encounters a low iron signal and stimulates the transcription of genes encoding the plasma membrane iron and siderophore transporters, the heme oxygenase (YLR205c) and the vacuolar iron transporter ( FET5/ FTH1).	gene_phenotype
71872	7	333683	11	NULL	NULL	0	NULL	statement 1	Process		occurs along with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_11_7762_s_216	11112771	In a frataxin-deficient strain mitochondrial free iron accumulates and cannot be extruded from mitochondria, so that Aft1p encounters a low iron signal and stimulates the transcription of genes encoding the plasma membrane iron and siderophore transporters, the heme oxygenase (YLR205c) and the vacuolar iron transporter ( FET5/ FTH1).	gene_phenotype
71873	8	333683	11	NULL	NULL	0	NULL	Aft1p	GP		encounters					low iron signal	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_11_7762_s_216	11112771	In a frataxin-deficient strain mitochondrial free iron accumulates and cannot be extruded from mitochondria, so that Aft1p encounters a low iron signal and stimulates the transcription of genes encoding the plasma membrane iron and siderophore transporters, the heme oxygenase (YLR205c) and the vacuolar iron transporter ( FET5/ FTH1).	gene_phenotype
71877	9	333683	11	NULL	NULL	0	NULL	statement 2	Process		leads to					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_11_7762_s_216	11112771	In a frataxin-deficient strain mitochondrial free iron accumulates and cannot be extruded from mitochondria, so that Aft1p encounters a low iron signal and stimulates the transcription of genes encoding the plasma membrane iron and siderophore transporters, the heme oxygenase (YLR205c) and the vacuolar iron transporter ( FET5/ FTH1).	gene_phenotype
71880	10	333683	11	NULL	NULL	0	NULL	statement 4	Process		stimulates					plasma membrane iron transporter gene	GP	transcription of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_11_7762_s_216	11112771	In a frataxin-deficient strain mitochondrial free iron accumulates and cannot be extruded from mitochondria, so that Aft1p encounters a low iron signal and stimulates the transcription of genes encoding the plasma membrane iron and siderophore transporters, the heme oxygenase (YLR205c) and the vacuolar iron transporter ( FET5/ FTH1).	gene_phenotype
71882	11	333683	11	NULL	NULL	0	NULL	statement 4	Process		stimulates					siderophore transporter gene	transcription of				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_11_7762_s_216	11112771	In a frataxin-deficient strain mitochondrial free iron accumulates and cannot be extruded from mitochondria, so that Aft1p encounters a low iron signal and stimulates the transcription of genes encoding the plasma membrane iron and siderophore transporters, the heme oxygenase (YLR205c) and the vacuolar iron transporter ( FET5/ FTH1).	gene_phenotype
70405	1	333687	11	NULL	NULL	0	NULL	Cin5	GP		undergoes					cellular localization	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_59_3_470_s_100	11179441	We examined the cellular localization of Cin5 and Ydr259c by inducing the expression of fusion proteins of Cin5 or Ydr259c with GFP in W303B cells (Fig.  5A).	gene_phenotype
70406	2	333687	11	NULL	NULL	0	NULL	Ydr259c	NucleicAcid		undergoes					cellular localization	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_59_3_470_s_100	11179441	We examined the cellular localization of Cin5 and Ydr259c by inducing the expression of fusion proteins of Cin5 or Ydr259c with GFP in W303B cells (Fig.  5A).	gene_phenotype
70407	3	333687	11	NULL	NULL	0	NULL	Cin5	GP		is a type of 					fusion protein	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_59_3_470_s_100	11179441	We examined the cellular localization of Cin5 and Ydr259c by inducing the expression of fusion proteins of Cin5 or Ydr259c with GFP in W303B cells (Fig.  5A).	gene_phenotype
70408	4	333687	11	NULL	NULL	0	NULL	Ydr259c	GP		is a type of 					fusion protein	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_59_3_470_s_100	11179441	We examined the cellular localization of Cin5 and Ydr259c by inducing the expression of fusion proteins of Cin5 or Ydr259c with GFP in W303B cells (Fig.  5A).	gene_phenotype
70409	5	333687	11	NULL	NULL	0	NULL	Cin5	GP		binds					GFP	GP				NULL	W303B cells	0	NULL	NULL	NULL	gw60_molpharmacol_59_3_470_s_100	11179441	We examined the cellular localization of Cin5 and Ydr259c by inducing the expression of fusion proteins of Cin5 or Ydr259c with GFP in W303B cells (Fig.  5A).	gene_phenotype
70410	6	333687	11	NULL	NULL	0	NULL	statement 5	Process		 induce the expression of					Cin5	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_59_3_470_s_100	11179441	We examined the cellular localization of Cin5 and Ydr259c by inducing the expression of fusion proteins of Cin5 or Ydr259c with GFP in W303B cells (Fig.  5A).	gene_phenotype
70411	7	333687	11	NULL	NULL	0	NULL	Ydr259c	NucleicAcid		binds					GFP	GP				NULL	 W303B cells	0	NULL	NULL	NULL	gw60_molpharmacol_59_3_470_s_100	11179441	We examined the cellular localization of Cin5 and Ydr259c by inducing the expression of fusion proteins of Cin5 or Ydr259c with GFP in W303B cells (Fig.  5A).	gene_phenotype
70412	8	333687	11	NULL	NULL	0	NULL	statement 7	Process		induce the expression of					Ydr259c	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_59_3_470_s_100	11179441	We examined the cellular localization of Cin5 and Ydr259c by inducing the expression of fusion proteins of Cin5 or Ydr259c with GFP in W303B cells (Fig.  5A).	gene_phenotype
70413	9	333687	11	NULL	NULL	0	NULL	statement 6	Process		induces					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_59_3_470_s_100	11179441	We examined the cellular localization of Cin5 and Ydr259c by inducing the expression of fusion proteins of Cin5 or Ydr259c with GFP in W303B cells (Fig.  5A).	gene_phenotype
70414	10	333687	11	NULL	NULL	0	NULL	statement 8	Process		induces					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_59_3_470_s_100	11179441	We examined the cellular localization of Cin5 and Ydr259c by inducing the expression of fusion proteins of Cin5 or Ydr259c with GFP in W303B cells (Fig.  5A).	gene_phenotype
70415	1	333688	11	NULL	NULL	0	NULL	 Cin5	GP		localized in the					nuclei	CellComponent	 yeast cell			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_59_3_470_s_8	11179441	An experiment with fusion proteins with green fluorescent protein revealed that Cin5 and Ydr259c were localized constitutively in the nuclei of yeast cells.	gene_phenotype
70416	2	333688	11	NULL	NULL	0	NULL	Ydr259c	GP		localized in the					 nuclei	CellComponent	yeast cell			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_59_3_470_s_8	11179441	An experiment with fusion proteins with green fluorescent protein revealed that Cin5 and Ydr259c were localized constitutively in the nuclei of yeast cells.	gene_phenotype
71892	1	333693	11	NULL	NULL	0	NULL	YOR193w	NucleicAcid		controls					peroxisome size	Cell Component				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_10_4089_s_261	14517321	These abnormally large peroxisomes could result from a disruption of components of the peroxisome division machinery in cells of the gene deletion strains, which is consistent with a role for  YOR193w in the control of peroxisome size, as has been proposed for  PEX25 and  PEX11 (Marshall  et al., 1995 ; Erdmann and Blobel, 1995 ; Smith  et al., 2002 ).	gene_phenotype
71894	2	333693	11	NULL	NULL	0	NULL	PEX25	GP		controls		possibly			peroxisome size	Cell Component				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_10_4089_s_261	14517321	These abnormally large peroxisomes could result from a disruption of components of the peroxisome division machinery in cells of the gene deletion strains, which is consistent with a role for  YOR193w in the control of peroxisome size, as has been proposed for  PEX25 and  PEX11 (Marshall  et al., 1995 ; Erdmann and Blobel, 1995 ; Smith  et al., 2002 ).	gene_phenotype
71896	3	333693	11	NULL	NULL	0	NULL	PEX11	GP		controls		possibly			peroxisome size	Cell Component				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_10_4089_s_261	14517321	These abnormally large peroxisomes could result from a disruption of components of the peroxisome division machinery in cells of the gene deletion strains, which is consistent with a role for  YOR193w in the control of peroxisome size, as has been proposed for  PEX25 and  PEX11 (Marshall  et al., 1995 ; Erdmann and Blobel, 1995 ; Smith  et al., 2002 ).	gene_phenotype
70417	1	333696	11	NULL	NULL	0	NULL	YGL133w	NucleicAcid	deletion	showed					abnormal morphology	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_336	14587103	In addition,   cells deleted in  YGL133w showed abnormal morphology (resembling the schmoo) and reduced mating efficiency  but, unlike the cell wall defects, these phenotypes were not observed when the  YGL133w disruption was in a  MAT a background (Escribano and Mazon, [ 2000]).	gene_phenotype
70418	2	333696	11	NULL	NULL	0	NULL	YGL133w	NucleicAcid	deletion	reduced					mating efficiency	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_336	14587103	In addition,   cells deleted in  YGL133w showed abnormal morphology (resembling the schmoo) and reduced mating efficiency  but, unlike the cell wall defects, these phenotypes were not observed when the  YGL133w disruption was in a  MAT a background (Escribano and Mazon, [ 2000]).	gene_phenotype
70419	1	333698	11	NULL	NULL	0	NULL	 YKR020w	NucleicAcid		 is essential for					Cvt vesicle formation	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_7_5009_s_4	12446664	We found that the  YKR020w gene product is essential for Cvt vesicle formation but not for pexophagy or induction of autophagy.	gene_phenotype
70420	2	333698	11	NULL	NULL	0	NULL	 YKR020w	NucleicAcid		is not essential for 					pexophagy	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_7_5009_s_4	12446664	We found that the  YKR020w gene product is essential for Cvt vesicle formation but not for pexophagy or induction of autophagy.	gene_phenotype
70421	3	333698	11	NULL	NULL	0	NULL	YKR020w	NucleicAcid		is not essential for 					autophagy	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_7_5009_s_4	12446664	We found that the  YKR020w gene product is essential for Cvt vesicle formation but not for pexophagy or induction of autophagy.	gene_phenotype
70422	1	333700	11	10	NULL	NULL	NULL	SIN3 gene	GP		 involved in					heterochromatin formation	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_4_1610_s_122	12686613	Mutation of  SIN3 or  SET2, genes involved in heterochromatin formation and gene silencing, completely suppressed the CPY secretion defect of the  vps51-1 strain but not that of  ykr020wdelta, suggesting that the upstream transposon insertion leads to transcriptional repression of  YKR020w (unpublished data).	gene_phenotype
70423	2	333700	11	10	NULL	NULL	NULL	SET2 gene	GP		 involved in					heterochromatin formation	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_4_1610_s_122	12686613	Mutation of  SIN3 or  SET2, genes involved in heterochromatin formation and gene silencing, completely suppressed the CPY secretion defect of the  vps51-1 strain but not that of  ykr020wdelta, suggesting that the upstream transposon insertion leads to transcriptional repression of  YKR020w (unpublished data).	gene_phenotype
70424	3	333700	11	10	NULL	NULL	NULL	SIN3 gene	GP		 involved in					gene silencing	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_4_1610_s_122	12686613	Mutation of  SIN3 or  SET2, genes involved in heterochromatin formation and gene silencing, completely suppressed the CPY secretion defect of the  vps51-1 strain but not that of  ykr020wdelta, suggesting that the upstream transposon insertion leads to transcriptional repression of  YKR020w (unpublished data).	gene_phenotype
70425	4	333700	11	10	NULL	NULL	NULL	SET2 gene	GP		involved in					gene silencing	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_4_1610_s_122	12686613	Mutation of  SIN3 or  SET2, genes involved in heterochromatin formation and gene silencing, completely suppressed the CPY secretion defect of the  vps51-1 strain but not that of  ykr020wdelta, suggesting that the upstream transposon insertion leads to transcriptional repression of  YKR020w (unpublished data).	gene_phenotype
70426	1	333701	11	NULL	NULL	NULL	NULL	YKR020w ORF	NucleicAcid	Deletion	secrets		increase			CPY 	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_14_4_1610_s_106	12686613	Deletion of the  YKR020w ORF gave rise to levels of CPY secretion and vacuolar morphology defects indistinguishable from those of the  vps51-1 mutant (compare Figures  1C and  2A), consistent with the results of a recent genome-wide screen for  vps mutants (Bonangelino  et al., 2002 ).	gene_phenotype
70427	2	333701	11	NULL	NULL	0	NULL	YKR020w ORF	NucleicAcid	deletion	defects					vacuolar morphology	CellComponent				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_14_4_1610_s_106	12686613	Deletion of the  YKR020w ORF gave rise to levels of CPY secretion and vacuolar morphology defects indistinguishable from those of the  vps51-1 mutant (compare Figures  1C and  2A), consistent with the results of a recent genome-wide screen for  vps mutants (Bonangelino  et al., 2002 ).	gene_phenotype
70428	1	333702	11	NULL	NULL	0	NULL	PDR16 gene	GP		involved in 					phospholipid synthesis	Process				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_gene_272_1-2_11470516_s_3	11470516	Among 20 genes containing binding consensus  sequences for the transcription factor Pdr1p in their promoter, we studied  more particularly the regulation and function of PDR16 (involved in phospholipid  synthesis), TPO1 (involved in vacuolar transport of polyamines), YAL061W  (homologous to polyol dehydrogenases) and YLR346C (unknown function).	gene_phenotype
70429	2	333702	11	NULL	NULL	0	NULL	TPO1 gene	GP		involved in					vacuolar transport	Process	of polyamines			NULL		0	NULL	NULL	NULL	abs-batch0517-0529_gene_272_1-2_11470516_s_3	11470516	Among 20 genes containing binding consensus  sequences for the transcription factor Pdr1p in their promoter, we studied  more particularly the regulation and function of PDR16 (involved in phospholipid  synthesis), TPO1 (involved in vacuolar transport of polyamines), YAL061W  (homologous to polyol dehydrogenases) and YLR346C (unknown function).	gene_phenotype
70430	3	333702	11	NULL	NULL	0	NULL	YAL061W gene	NucleicAcid		homologous to					polyol dehydrogenase	GP				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_gene_272_1-2_11470516_s_3	11470516	Among 20 genes containing binding consensus  sequences for the transcription factor Pdr1p in their promoter, we studied  more particularly the regulation and function of PDR16 (involved in phospholipid  synthesis), TPO1 (involved in vacuolar transport of polyamines), YAL061W  (homologous to polyol dehydrogenases) and YLR346C (unknown function).	gene_phenotype
70431	1	333703	11	NULL	NULL	0	NULL	YOR249c ORF	NucleicAcid	Deletion	reduces					viability	Process				NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1219_s_50	9469815	Deletion of this ORF from the  S. cerevisiae genome indicates that YOR249c is essential for viability, and the null mutants exhibit a terminal G2-M arrest phenotype as would be expected for APC genes ( 23).	gene_phenotype
70432	2	333703	11	NULL	NULL	0	NULL	 YOR249c ORF 	NucleicAcid	null mutant	exhibit					G2-M arrest	Process	terminal			NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1219_s_50	9469815	Deletion of this ORF from the  S. cerevisiae genome indicates that YOR249c is essential for viability, and the null mutants exhibit a terminal G2-M arrest phenotype as would be expected for APC genes ( 23).	gene_phenotype
70433	3	333703	11	NULL	NULL	0	NULL	APC gene	GP		exhibit					G2-M arrest	Process	terminal			NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1219_s_50	9469815	Deletion of this ORF from the  S. cerevisiae genome indicates that YOR249c is essential for viability, and the null mutants exhibit a terminal G2-M arrest phenotype as would be expected for APC genes ( 23).	gene_phenotype
70434	1	333705	11	NULL	NULL	0	NULL	 Crn1	GP		is a type of 					actin-bundling protein	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_154_3_549_s_328	11489916	Ynl094w also interacted with the actin-bundling protein Crn1 ( Goode et al., 1999) and with Sro77, a protein which functions in polarized secretion ( Kagami et al., 1998;  Lehman et al., 1999).	gene_phenotype
70435	2	333705	11	NULL	NULL	0	NULL	Sro77	GP		 functions in					polarized secretion	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_154_3_549_s_328	11489916	Ynl094w also interacted with the actin-bundling protein Crn1 ( Goode et al., 1999) and with Sro77, a protein which functions in polarized secretion ( Kagami et al., 1998;  Lehman et al., 1999).	gene_phenotype
70436	3	333705	11	NULL	NULL	NULL	NULL	Ynl094w	NucleicAcid		interacts with 					Crn1	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_154_3_549_s_328	11489916	Ynl094w also interacted with the actin-bundling protein Crn1 ( Goode et al., 1999) and with Sro77, a protein which functions in polarized secretion ( Kagami et al., 1998;  Lehman et al., 1999).	gene_phenotype
70437	4	333705	11	NULL	NULL	0	NULL	Ynl094w	GP		interacts with 					Sro77	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_154_3_549_s_328	11489916	Ynl094w also interacted with the actin-bundling protein Crn1 ( Goode et al., 1999) and with Sro77, a protein which functions in polarized secretion ( Kagami et al., 1998;  Lehman et al., 1999).	gene_phenotype
70438	1	333707	11	NULL	NULL	0	NULL	COS12 gene	GP		derepress					 telomeric silencing	Process				NULL		0	NULL	NULL	NULL	gw60_science_285_5427_591_s_100	10417390	Furthermore, transcription of a number of genes located very near telomeres, including  COS12,  YER188W, and  YAL069W, increased 1.6- to 2.5-fold, consistent with derepression of telomeric silencing.	gene_phenotype
70439	2	333707	11	NULL	NULL	0	NULL	YER188W gene	NucleicAcid		derepress					telomeric silencing	Process				NULL		0	NULL	NULL	NULL	gw60_science_285_5427_591_s_100	10417390	Furthermore, transcription of a number of genes located very near telomeres, including  COS12,  YER188W, and  YAL069W, increased 1.6- to 2.5-fold, consistent with derepression of telomeric silencing.	gene_phenotype
70440	3	333707	11	NULL	NULL	0	NULL	YAL069W gene	NucleicAcid		derepress					telomeric silencing	Process				NULL		0	NULL	NULL	NULL	gw60_science_285_5427_591_s_100	10417390	Furthermore, transcription of a number of genes located very near telomeres, including  COS12,  YER188W, and  YAL069W, increased 1.6- to 2.5-fold, consistent with derepression of telomeric silencing.	gene_phenotype
70441	1	333708	11	NULL	NULL	0	NULL	 YHR076w gene	NucleicAcid		encodes					 type 2C protein phosphatase	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_20_2_185_s_576	12568102	The  YHR076w gene encodes a type 2C protein phosphatase and represents the seventh PP2C gene in  budding yeast (Letter).	gene_phenotype
70442	2	333708	11	NULL	NULL	0	NULL	YHR076w gene	NucleicAcid		 represents					seventh PP2C gene	GP	budding yeast			NULL		0	NULL	NULL	NULL	gw70_yeast_20_2_185_s_576	12568102	The  YHR076w gene encodes a type 2C protein phosphatase and represents the seventh PP2C gene in  budding yeast (Letter).	gene_phenotype
70443	1	333710	11	NULL	NULL	0	NULL	PGU1	GP		is a type of 					secreted protein	GP				NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_306	10657304	Genes encoding secreted proteins ( PGU1 and  PRY2), potential cell-surface proteins ( YLR042c,  YIL117c), proteins involved in glycosylation and chitin biosynthesis ( KTR2,  CHS7, and  GFA1), and a regulatory protein implicated in invasive and filamentous growth ( PHD1) were all induced by Kss1p signaling.	gene_phenotype
70444	2	333710	11	NULL	NULL	0	NULL	 PRY2	GP		is a type of 					secreted proteins	GP				NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_306	10657304	Genes encoding secreted proteins ( PGU1 and  PRY2), potential cell-surface proteins ( YLR042c,  YIL117c), proteins involved in glycosylation and chitin biosynthesis ( KTR2,  CHS7, and  GFA1), and a regulatory protein implicated in invasive and filamentous growth ( PHD1) were all induced by Kss1p signaling.	gene_phenotype
70445	3	333710	11	NULL	NULL	0	NULL	YLR042c	NucleicAcid		is a type of 					cell-surface protein	GP				NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_306	10657304	Genes encoding secreted proteins ( PGU1 and  PRY2), potential cell-surface proteins ( YLR042c,  YIL117c), proteins involved in glycosylation and chitin biosynthesis ( KTR2,  CHS7, and  GFA1), and a regulatory protein implicated in invasive and filamentous growth ( PHD1) were all induced by Kss1p signaling.	gene_phenotype
70446	4	333710	11	NULL	NULL	0	NULL	YIL117c	NucleicAcid		is a type of 					cell-surface protein	GP				NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_306	10657304	Genes encoding secreted proteins ( PGU1 and  PRY2), potential cell-surface proteins ( YLR042c,  YIL117c), proteins involved in glycosylation and chitin biosynthesis ( KTR2,  CHS7, and  GFA1), and a regulatory protein implicated in invasive and filamentous growth ( PHD1) were all induced by Kss1p signaling.	gene_phenotype
70447	5	333710	11	NULL	NULL	0	NULL	chitin	Chemical		undergoes					biosynthesis	Process				NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_306	10657304	Genes encoding secreted proteins ( PGU1 and  PRY2), potential cell-surface proteins ( YLR042c,  YIL117c), proteins involved in glycosylation and chitin biosynthesis ( KTR2,  CHS7, and  GFA1), and a regulatory protein implicated in invasive and filamentous growth ( PHD1) were all induced by Kss1p signaling.	gene_phenotype
70448	6	333710	11	NULL	NULL	0	NULL	 KTR2	GP		involved in					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_306	10657304	Genes encoding secreted proteins ( PGU1 and  PRY2), potential cell-surface proteins ( YLR042c,  YIL117c), proteins involved in glycosylation and chitin biosynthesis ( KTR2,  CHS7, and  GFA1), and a regulatory protein implicated in invasive and filamentous growth ( PHD1) were all induced by Kss1p signaling.	gene_phenotype
70449	7	333710	11	NULL	NULL	0	NULL	CHS7	GP		involved in					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_306	10657304	Genes encoding secreted proteins ( PGU1 and  PRY2), potential cell-surface proteins ( YLR042c,  YIL117c), proteins involved in glycosylation and chitin biosynthesis ( KTR2,  CHS7, and  GFA1), and a regulatory protein implicated in invasive and filamentous growth ( PHD1) were all induced by Kss1p signaling.	gene_phenotype
70450	8	333710	11	NULL	NULL	0	NULL	GFA1	GP		involved in					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_306	10657304	Genes encoding secreted proteins ( PGU1 and  PRY2), potential cell-surface proteins ( YLR042c,  YIL117c), proteins involved in glycosylation and chitin biosynthesis ( KTR2,  CHS7, and  GFA1), and a regulatory protein implicated in invasive and filamentous growth ( PHD1) were all induced by Kss1p signaling.	gene_phenotype
70451	9	333710	11	NULL	NULL	0	NULL	PHD1	GP		is a type of 					filamentous growth protien	GP				NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_306	10657304	Genes encoding secreted proteins ( PGU1 and  PRY2), potential cell-surface proteins ( YLR042c,  YIL117c), proteins involved in glycosylation and chitin biosynthesis ( KTR2,  CHS7, and  GFA1), and a regulatory protein implicated in invasive and filamentous growth ( PHD1) were all induced by Kss1p signaling.	gene_phenotype
70452	10	333710	11	NULL	NULL	0	NULL	Kss1p	GP	signaling	induced					PGU1	GP				NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_306	10657304	Genes encoding secreted proteins ( PGU1 and  PRY2), potential cell-surface proteins ( YLR042c,  YIL117c), proteins involved in glycosylation and chitin biosynthesis ( KTR2,  CHS7, and  GFA1), and a regulatory protein implicated in invasive and filamentous growth ( PHD1) were all induced by Kss1p signaling.	gene_phenotype
70453	11	333710	11	NULL	NULL	0	NULL	Kss1p	GP	signaling	induced					PRY2	GP				NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_306	10657304	Genes encoding secreted proteins ( PGU1 and  PRY2), potential cell-surface proteins ( YLR042c,  YIL117c), proteins involved in glycosylation and chitin biosynthesis ( KTR2,  CHS7, and  GFA1), and a regulatory protein implicated in invasive and filamentous growth ( PHD1) were all induced by Kss1p signaling.	gene_phenotype
70454	12	333710	11	NULL	NULL	0	NULL	 Kss1p	GP	signaling	induced					YLR042c	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_306	10657304	Genes encoding secreted proteins ( PGU1 and  PRY2), potential cell-surface proteins ( YLR042c,  YIL117c), proteins involved in glycosylation and chitin biosynthesis ( KTR2,  CHS7, and  GFA1), and a regulatory protein implicated in invasive and filamentous growth ( PHD1) were all induced by Kss1p signaling.	gene_phenotype
70455	13	333710	11	NULL	NULL	0	NULL	Kss1p	GP	signaling	induced					YIL117c	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_306	10657304	Genes encoding secreted proteins ( PGU1 and  PRY2), potential cell-surface proteins ( YLR042c,  YIL117c), proteins involved in glycosylation and chitin biosynthesis ( KTR2,  CHS7, and  GFA1), and a regulatory protein implicated in invasive and filamentous growth ( PHD1) were all induced by Kss1p signaling.	gene_phenotype
70456	14	333710	11	NULL	NULL	0	NULL	Kss1p	GP	signaling	induced					 KTR2	GP				NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_306	10657304	Genes encoding secreted proteins ( PGU1 and  PRY2), potential cell-surface proteins ( YLR042c,  YIL117c), proteins involved in glycosylation and chitin biosynthesis ( KTR2,  CHS7, and  GFA1), and a regulatory protein implicated in invasive and filamentous growth ( PHD1) were all induced by Kss1p signaling.	gene_phenotype
70457	15	333710	11	NULL	NULL	0	NULL	Kss1p	GP	signaling	induced					CHS7	GP				NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_306	10657304	Genes encoding secreted proteins ( PGU1 and  PRY2), potential cell-surface proteins ( YLR042c,  YIL117c), proteins involved in glycosylation and chitin biosynthesis ( KTR2,  CHS7, and  GFA1), and a regulatory protein implicated in invasive and filamentous growth ( PHD1) were all induced by Kss1p signaling.	gene_phenotype
70458	16	333710	11	NULL	NULL	0	NULL	Kss1p	GP	signaling	induced					GFA1	GP				NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_306	10657304	Genes encoding secreted proteins ( PGU1 and  PRY2), potential cell-surface proteins ( YLR042c,  YIL117c), proteins involved in glycosylation and chitin biosynthesis ( KTR2,  CHS7, and  GFA1), and a regulatory protein implicated in invasive and filamentous growth ( PHD1) were all induced by Kss1p signaling.	gene_phenotype
70459	17	333710	11	NULL	NULL	0	NULL	Kss1p	GP	signaling	induced					PHD1	GP				NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_306	10657304	Genes encoding secreted proteins ( PGU1 and  PRY2), potential cell-surface proteins ( YLR042c,  YIL117c), proteins involved in glycosylation and chitin biosynthesis ( KTR2,  CHS7, and  GFA1), and a regulatory protein implicated in invasive and filamentous growth ( PHD1) were all induced by Kss1p signaling.	gene_phenotype
70460	1	333713	11	NULL	NULL	0	NULL	YML059c	NucleicAcid		activates					Serine Esterase	GP	OP-sensitive			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24024_s_100	15044461	YML059c Has OP-sensitive Serine Esterase Activity and Can Deacylate Exogenous Lysophospholipid -- Sequence similarity between YML059c and NTE (39% identity in the catalytic domain; see  Fig. 2 a and alignments in Ref.  ) strongly suggest that the yeast protein may have serine esterase activity.	gene_phenotype
70461	2	333713	11	NULL	NULL	0	NULL	YML059c	NucleicAcid		Deacylate					Lysophospholipid	Chemical	Exogenous			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24024_s_100	15044461	YML059c Has OP-sensitive Serine Esterase Activity and Can Deacylate Exogenous Lysophospholipid -- Sequence similarity between YML059c and NTE (39% identity in the catalytic domain; see  Fig. 2 a and alignments in Ref.  ) strongly suggest that the yeast protein may have serine esterase activity.	gene_phenotype
70462	1	333718	11	NULL	NULL	0	NULL	 transporter protein 	GP		intake					Cho	Chemical	Extracellular			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24024_s_17	15044461	Extracellular Cho is taken up into the cell by a transporter protein ( 1) and phosphorylated via choline kinase ( 2);  3, phosphocholine ( PCho) is condenses with CTP in the rate-limiting step for PtdCho synthesis mediated by  CTP-phosphocholine cytidylyltransferase ( CCT);  4, CDP-choline reacts with diacylglycerol catalyzed by choline phosphotransferase;   5, PtdCho can be hydrolyzed by phospholipase D, forming phosphatidic acid and Cho;  the latter can be phosphorylated ( step 2) or secreted ( step 6) from the cell;  7, PtdCho is deacylated at both sn-2 and sn-1 positions to yield GroPCho and two molecules  of free fatty acid; we show here that this deacylation is mediated by NTE in mammalian  cells and by its homologue, YML059c, in yeast.	gene_phenotype
70463	2	333718	11	NULL	NULL	0	NULL	choline kinase	GP		phosphorylates					Cho	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24024_s_17	15044461	Extracellular Cho is taken up into the cell by a transporter protein ( 1) and phosphorylated via choline kinase ( 2);  3, phosphocholine ( PCho) is condenses with CTP in the rate-limiting step for PtdCho synthesis mediated by  CTP-phosphocholine cytidylyltransferase ( CCT);  4, CDP-choline reacts with diacylglycerol catalyzed by choline phosphotransferase;   5, PtdCho can be hydrolyzed by phospholipase D, forming phosphatidic acid and Cho;  the latter can be phosphorylated ( step 2) or secreted ( step 6) from the cell;  7, PtdCho is deacylated at both sn-2 and sn-1 positions to yield GroPCho and two molecules  of free fatty acid; we show here that this deacylation is mediated by NTE in mammalian  cells and by its homologue, YML059c, in yeast.	gene_phenotype
70464	3	333718	11	NULL	NULL	0	NULL	CCT	GP		is					CTP-phosphocholine cytidylyltransferase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24024_s_17	15044461	Extracellular Cho is taken up into the cell by a transporter protein ( 1) and phosphorylated via choline kinase ( 2);  3, phosphocholine ( PCho) is condenses with CTP in the rate-limiting step for PtdCho synthesis mediated by  CTP-phosphocholine cytidylyltransferase ( CCT);  4, CDP-choline reacts with diacylglycerol catalyzed by choline phosphotransferase;   5, PtdCho can be hydrolyzed by phospholipase D, forming phosphatidic acid and Cho;  the latter can be phosphorylated ( step 2) or secreted ( step 6) from the cell;  7, PtdCho is deacylated at both sn-2 and sn-1 positions to yield GroPCho and two molecules  of free fatty acid; we show here that this deacylation is mediated by NTE in mammalian  cells and by its homologue, YML059c, in yeast.	gene_phenotype
70465	4	333718	11	NULL	NULL	0	NULL	CTP-phosphocholine cytidylyltransferase	GP		synthesises					PtdCho	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24024_s_17	15044461	Extracellular Cho is taken up into the cell by a transporter protein ( 1) and phosphorylated via choline kinase ( 2);  3, phosphocholine ( PCho) is condenses with CTP in the rate-limiting step for PtdCho synthesis mediated by  CTP-phosphocholine cytidylyltransferase ( CCT);  4, CDP-choline reacts with diacylglycerol catalyzed by choline phosphotransferase;   5, PtdCho can be hydrolyzed by phospholipase D, forming phosphatidic acid and Cho;  the latter can be phosphorylated ( step 2) or secreted ( step 6) from the cell;  7, PtdCho is deacylated at both sn-2 and sn-1 positions to yield GroPCho and two molecules  of free fatty acid; we show here that this deacylation is mediated by NTE in mammalian  cells and by its homologue, YML059c, in yeast.	gene_phenotype
70466	5	333718	11	NULL	NULL	0	NULL	CDP-choline	Chemical		 reacts with					diacylglycerol	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24024_s_17	15044461	Extracellular Cho is taken up into the cell by a transporter protein ( 1) and phosphorylated via choline kinase ( 2);  3, phosphocholine ( PCho) is condenses with CTP in the rate-limiting step for PtdCho synthesis mediated by  CTP-phosphocholine cytidylyltransferase ( CCT);  4, CDP-choline reacts with diacylglycerol catalyzed by choline phosphotransferase;   5, PtdCho can be hydrolyzed by phospholipase D, forming phosphatidic acid and Cho;  the latter can be phosphorylated ( step 2) or secreted ( step 6) from the cell;  7, PtdCho is deacylated at both sn-2 and sn-1 positions to yield GroPCho and two molecules  of free fatty acid; we show here that this deacylation is mediated by NTE in mammalian  cells and by its homologue, YML059c, in yeast.	gene_phenotype
70467	6	333718	11	NULL	NULL	0	NULL	statement 5	Process		catalyzed by					choline phosphotransferase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24024_s_17	15044461	Extracellular Cho is taken up into the cell by a transporter protein ( 1) and phosphorylated via choline kinase ( 2);  3, phosphocholine ( PCho) is condenses with CTP in the rate-limiting step for PtdCho synthesis mediated by  CTP-phosphocholine cytidylyltransferase ( CCT);  4, CDP-choline reacts with diacylglycerol catalyzed by choline phosphotransferase;   5, PtdCho can be hydrolyzed by phospholipase D, forming phosphatidic acid and Cho;  the latter can be phosphorylated ( step 2) or secreted ( step 6) from the cell;  7, PtdCho is deacylated at both sn-2 and sn-1 positions to yield GroPCho and two molecules  of free fatty acid; we show here that this deacylation is mediated by NTE in mammalian  cells and by its homologue, YML059c, in yeast.	gene_phenotype
70468	7	333718	11	NULL	NULL	0	NULL	 phospholipase D	GP		hydrolyzes 					PtdCho	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24024_s_17	15044461	Extracellular Cho is taken up into the cell by a transporter protein ( 1) and phosphorylated via choline kinase ( 2);  3, phosphocholine ( PCho) is condenses with CTP in the rate-limiting step for PtdCho synthesis mediated by  CTP-phosphocholine cytidylyltransferase ( CCT);  4, CDP-choline reacts with diacylglycerol catalyzed by choline phosphotransferase;   5, PtdCho can be hydrolyzed by phospholipase D, forming phosphatidic acid and Cho;  the latter can be phosphorylated ( step 2) or secreted ( step 6) from the cell;  7, PtdCho is deacylated at both sn-2 and sn-1 positions to yield GroPCho and two molecules  of free fatty acid; we show here that this deacylation is mediated by NTE in mammalian  cells and by its homologue, YML059c, in yeast.	gene_phenotype
70469	8	333718	11	NULL	NULL	0	NULL	statement 7	Process		forms					phosphatidic acid	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24024_s_17	15044461	Extracellular Cho is taken up into the cell by a transporter protein ( 1) and phosphorylated via choline kinase ( 2);  3, phosphocholine ( PCho) is condenses with CTP in the rate-limiting step for PtdCho synthesis mediated by  CTP-phosphocholine cytidylyltransferase ( CCT);  4, CDP-choline reacts with diacylglycerol catalyzed by choline phosphotransferase;   5, PtdCho can be hydrolyzed by phospholipase D, forming phosphatidic acid and Cho;  the latter can be phosphorylated ( step 2) or secreted ( step 6) from the cell;  7, PtdCho is deacylated at both sn-2 and sn-1 positions to yield GroPCho and two molecules  of free fatty acid; we show here that this deacylation is mediated by NTE in mammalian  cells and by its homologue, YML059c, in yeast.	gene_phenotype
70470	9	333718	11	NULL	NULL	0	NULL	statement 7	Process		forms					Cho	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24024_s_17	15044461	Extracellular Cho is taken up into the cell by a transporter protein ( 1) and phosphorylated via choline kinase ( 2);  3, phosphocholine ( PCho) is condenses with CTP in the rate-limiting step for PtdCho synthesis mediated by  CTP-phosphocholine cytidylyltransferase ( CCT);  4, CDP-choline reacts with diacylglycerol catalyzed by choline phosphotransferase;   5, PtdCho can be hydrolyzed by phospholipase D, forming phosphatidic acid and Cho;  the latter can be phosphorylated ( step 2) or secreted ( step 6) from the cell;  7, PtdCho is deacylated at both sn-2 and sn-1 positions to yield GroPCho and two molecules  of free fatty acid; we show here that this deacylation is mediated by NTE in mammalian  cells and by its homologue, YML059c, in yeast.	gene_phenotype
70471	10	333718	11	NULL	NULL	0	NULL	statement 8	Process		occurs along with					statement 9	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24024_s_17	15044461	Extracellular Cho is taken up into the cell by a transporter protein ( 1) and phosphorylated via choline kinase ( 2);  3, phosphocholine ( PCho) is condenses with CTP in the rate-limiting step for PtdCho synthesis mediated by  CTP-phosphocholine cytidylyltransferase ( CCT);  4, CDP-choline reacts with diacylglycerol catalyzed by choline phosphotransferase;   5, PtdCho can be hydrolyzed by phospholipase D, forming phosphatidic acid and Cho;  the latter can be phosphorylated ( step 2) or secreted ( step 6) from the cell;  7, PtdCho is deacylated at both sn-2 and sn-1 positions to yield GroPCho and two molecules  of free fatty acid; we show here that this deacylation is mediated by NTE in mammalian  cells and by its homologue, YML059c, in yeast.	gene_phenotype
70472	11	333718	11	NULL	NULL	0	NULL	Cho	Chemical		undergoes					phosphorylation	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24024_s_17	15044461	Extracellular Cho is taken up into the cell by a transporter protein ( 1) and phosphorylated via choline kinase ( 2);  3, phosphocholine ( PCho) is condenses with CTP in the rate-limiting step for PtdCho synthesis mediated by  CTP-phosphocholine cytidylyltransferase ( CCT);  4, CDP-choline reacts with diacylglycerol catalyzed by choline phosphotransferase;   5, PtdCho can be hydrolyzed by phospholipase D, forming phosphatidic acid and Cho;  the latter can be phosphorylated ( step 2) or secreted ( step 6) from the cell;  7, PtdCho is deacylated at both sn-2 and sn-1 positions to yield GroPCho and two molecules  of free fatty acid; we show here that this deacylation is mediated by NTE in mammalian  cells and by its homologue, YML059c, in yeast.	gene_phenotype
70473	12	333718	11	NULL	NULL	0	NULL	Cho	Chemical		undergoes					Secretion 	Process	 from the cell			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24024_s_17	15044461	Extracellular Cho is taken up into the cell by a transporter protein ( 1) and phosphorylated via choline kinase ( 2);  3, phosphocholine ( PCho) is condenses with CTP in the rate-limiting step for PtdCho synthesis mediated by  CTP-phosphocholine cytidylyltransferase ( CCT);  4, CDP-choline reacts with diacylglycerol catalyzed by choline phosphotransferase;   5, PtdCho can be hydrolyzed by phospholipase D, forming phosphatidic acid and Cho;  the latter can be phosphorylated ( step 2) or secreted ( step 6) from the cell;  7, PtdCho is deacylated at both sn-2 and sn-1 positions to yield GroPCho and two molecules  of free fatty acid; we show here that this deacylation is mediated by NTE in mammalian  cells and by its homologue, YML059c, in yeast.	gene_phenotype
70474	13	333718	11	NULL	NULL	0	NULL	PtdCho	Chemical		undergoes					deacylation	Process	at sn-2 and sn-1 positions			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24024_s_17	15044461	Extracellular Cho is taken up into the cell by a transporter protein ( 1) and phosphorylated via choline kinase ( 2);  3, phosphocholine ( PCho) is condenses with CTP in the rate-limiting step for PtdCho synthesis mediated by  CTP-phosphocholine cytidylyltransferase ( CCT);  4, CDP-choline reacts with diacylglycerol catalyzed by choline phosphotransferase;   5, PtdCho can be hydrolyzed by phospholipase D, forming phosphatidic acid and Cho;  the latter can be phosphorylated ( step 2) or secreted ( step 6) from the cell;  7, PtdCho is deacylated at both sn-2 and sn-1 positions to yield GroPCho and two molecules  of free fatty acid; we show here that this deacylation is mediated by NTE in mammalian  cells and by its homologue, YML059c, in yeast.	gene_phenotype
70475	14	333718	11	NULL	NULL	0	NULL	statement 13	Process		 yield					GroPCho	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24024_s_17	15044461	Extracellular Cho is taken up into the cell by a transporter protein ( 1) and phosphorylated via choline kinase ( 2);  3, phosphocholine ( PCho) is condenses with CTP in the rate-limiting step for PtdCho synthesis mediated by  CTP-phosphocholine cytidylyltransferase ( CCT);  4, CDP-choline reacts with diacylglycerol catalyzed by choline phosphotransferase;   5, PtdCho can be hydrolyzed by phospholipase D, forming phosphatidic acid and Cho;  the latter can be phosphorylated ( step 2) or secreted ( step 6) from the cell;  7, PtdCho is deacylated at both sn-2 and sn-1 positions to yield GroPCho and two molecules  of free fatty acid; we show here that this deacylation is mediated by NTE in mammalian  cells and by its homologue, YML059c, in yeast.	gene_phenotype
70476	15	333718	11	NULL	NULL	0	NULL	statement 13	Process		 yield					free fatty acid	Chemical	two molecules			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24024_s_17	15044461	Extracellular Cho is taken up into the cell by a transporter protein ( 1) and phosphorylated via choline kinase ( 2);  3, phosphocholine ( PCho) is condenses with CTP in the rate-limiting step for PtdCho synthesis mediated by  CTP-phosphocholine cytidylyltransferase ( CCT);  4, CDP-choline reacts with diacylglycerol catalyzed by choline phosphotransferase;   5, PtdCho can be hydrolyzed by phospholipase D, forming phosphatidic acid and Cho;  the latter can be phosphorylated ( step 2) or secreted ( step 6) from the cell;  7, PtdCho is deacylated at both sn-2 and sn-1 positions to yield GroPCho and two molecules  of free fatty acid; we show here that this deacylation is mediated by NTE in mammalian  cells and by its homologue, YML059c, in yeast.	gene_phenotype
70477	16	333718	11	NULL	NULL	0	NULL	statement 14	Process		occurs along with					statement 15	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24024_s_17	15044461	Extracellular Cho is taken up into the cell by a transporter protein ( 1) and phosphorylated via choline kinase ( 2);  3, phosphocholine ( PCho) is condenses with CTP in the rate-limiting step for PtdCho synthesis mediated by  CTP-phosphocholine cytidylyltransferase ( CCT);  4, CDP-choline reacts with diacylglycerol catalyzed by choline phosphotransferase;   5, PtdCho can be hydrolyzed by phospholipase D, forming phosphatidic acid and Cho;  the latter can be phosphorylated ( step 2) or secreted ( step 6) from the cell;  7, PtdCho is deacylated at both sn-2 and sn-1 positions to yield GroPCho and two molecules  of free fatty acid; we show here that this deacylation is mediated by NTE in mammalian  cells and by its homologue, YML059c, in yeast.	gene_phenotype
70478	17	333718	11	NULL	NULL	0	NULL	NTE	GP	mammalian cells	mediate					statement 13	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24024_s_17	15044461	Extracellular Cho is taken up into the cell by a transporter protein ( 1) and phosphorylated via choline kinase ( 2);  3, phosphocholine ( PCho) is condenses with CTP in the rate-limiting step for PtdCho synthesis mediated by  CTP-phosphocholine cytidylyltransferase ( CCT);  4, CDP-choline reacts with diacylglycerol catalyzed by choline phosphotransferase;   5, PtdCho can be hydrolyzed by phospholipase D, forming phosphatidic acid and Cho;  the latter can be phosphorylated ( step 2) or secreted ( step 6) from the cell;  7, PtdCho is deacylated at both sn-2 and sn-1 positions to yield GroPCho and two molecules  of free fatty acid; we show here that this deacylation is mediated by NTE in mammalian  cells and by its homologue, YML059c, in yeast.	gene_phenotype
70479	18	333718	11	NULL	NULL	0	NULL	YML059c	NucleicAcid	yeast	mediate					statement 13	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24024_s_17	15044461	Extracellular Cho is taken up into the cell by a transporter protein ( 1) and phosphorylated via choline kinase ( 2);  3, phosphocholine ( PCho) is condenses with CTP in the rate-limiting step for PtdCho synthesis mediated by  CTP-phosphocholine cytidylyltransferase ( CCT);  4, CDP-choline reacts with diacylglycerol catalyzed by choline phosphotransferase;   5, PtdCho can be hydrolyzed by phospholipase D, forming phosphatidic acid and Cho;  the latter can be phosphorylated ( step 2) or secreted ( step 6) from the cell;  7, PtdCho is deacylated at both sn-2 and sn-1 positions to yield GroPCho and two molecules  of free fatty acid; we show here that this deacylation is mediated by NTE in mammalian  cells and by its homologue, YML059c, in yeast.	gene_phenotype
70480	19	333718	11	NULL	NULL	0	NULL	YML059c	NucleicAcid	yeast	is a  homologue of					NTE	GP	mammalian cell			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_23_24024_s_17	15044461	Extracellular Cho is taken up into the cell by a transporter protein ( 1) and phosphorylated via choline kinase ( 2);  3, phosphocholine ( PCho) is condenses with CTP in the rate-limiting step for PtdCho synthesis mediated by  CTP-phosphocholine cytidylyltransferase ( CCT);  4, CDP-choline reacts with diacylglycerol catalyzed by choline phosphotransferase;   5, PtdCho can be hydrolyzed by phospholipase D, forming phosphatidic acid and Cho;  the latter can be phosphorylated ( step 2) or secreted ( step 6) from the cell;  7, PtdCho is deacylated at both sn-2 and sn-1 positions to yield GroPCho and two molecules  of free fatty acid; we show here that this deacylation is mediated by NTE in mammalian  cells and by its homologue, YML059c, in yeast.	gene_phenotype
71874	1	333725	11	NULL	NULL	NULL	NULL	Sac1p-like protein	GP	Budding yeast	 regulate		possibly			PI(3)P levels	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_16_8910_s_150	10900271	Budding yeast express several Sac1p-like proteins, as well as a PTEN-like phosphatase (YNL128w), which are also thought to play a role in regulating PI(3)P levels ( 36,  37).	gene_phenotype
71875	2	333725	11	NULL	NULL	0	NULL	PTEN-like phosphatase	GP	Budding yeast	regulate		possibly			PI(3)P levels	Chemical				NULL		0	NULL	NULL	NULL	gw60_pnas_97_16_8910_s_150	10900271	Budding yeast express several Sac1p-like proteins, as well as a PTEN-like phosphatase (YNL128w), which are also thought to play a role in regulating PI(3)P levels ( 36,  37).	gene_phenotype
71876	3	333725	11	NULL	NULL	0	NULL	YNL128w	NucleicAcid		is a synonym of					PTEN-like phosphatase	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_97_16_8910_s_150	10900271	Budding yeast express several Sac1p-like proteins, as well as a PTEN-like phosphatase (YNL128w), which are also thought to play a role in regulating PI(3)P levels ( 36,  37).	gene_phenotype
69705	1	333726	5	NULL	NULL	0	NULL	YNL128w	NucleicAcid		plays a role in		may			sporulation	Process				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_70_0_247_s_329	11395408	A single report has demonstrated that YNL128w is one of  158 genes whose expression is induced from 2 to 5 hours after transfer to sporulation  medium during the completion of meiotic prophase, which suggests it may play a role  in sporulation ( 107).	gene_phenotype
69710	1	333728	5	NULL	NULL	0	NULL	YLR109W	NucleicAcid		activates					tert-butyl hydroperoxide 2	Chemical	defense against			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_35_22480_s_220	9712873	YLR109W displays defense activity against  tert-butyl hydroperoxide 2 and represents a subclass of the AhpC/TSA protein family localized in the peroxisome.	gene_phenotype
69711	2	333728	5	NULL	NULL	0	NULL	AhpC/TSA protein family	GP		is localized in					peroxisome	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_35_22480_s_220	9712873	YLR109W displays defense activity against  tert-butyl hydroperoxide 2 and represents a subclass of the AhpC/TSA protein family localized in the peroxisome.	gene_phenotype
69714	3	333728	5	NULL	NULL	0	NULL	YLR109W	NucleicAcid		represent					AhpC/TSA protein family	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_35_22480_s_220	9712873	YLR109W displays defense activity against  tert-butyl hydroperoxide 2 and represents a subclass of the AhpC/TSA protein family localized in the peroxisome.	gene_phenotype
69716	1	333730	5	NULL	NULL	0	NULL	YOL095c protein	GP		is located in					mitochondria	CellComponent	yeast			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_5_1816_s_23	10669756	The YOL095c protein is located in yeast mitochondria, and is required for wild-type (wt) [ rho+] mitochondrial genome maintenance.	gene_phenotype
69717	2	333730	5	NULL	NULL	0	NULL	YOL095c protein	GP		is required for					genome maintenance	Process	wild-type;;[ rho+] mitochondria			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_5_1816_s_23	10669756	The YOL095c protein is located in yeast mitochondria, and is required for wild-type (wt) [ rho+] mitochondrial genome maintenance.	gene_phenotype
69725	1	333733	5	NULL	NULL	0	NULL	YIL113w disruptant strain	Organism		responds to		normally			mating pheromone	Chemical				NULL		0	NULL	NULL	NULL	gw60_febslett_527_1_186_s_190	12220658	This conclusion is supported by our own findings in which a  YIL113w disruptant strain exhibited a normal response to mating pheromone, indicating that Yil113p is not involved in regulating the Fus3p MAPK (M.C., unpublished observations) and by the results of a study in which disruption of  YIL113w alone or in combination with  PTP2 and/or  MSG5 was found to have no effect on phosphorylation of the Hog1p MAPK, indicating that Yil113p is not involved in regulating the response to osmotic stress in  S. cerevisiae [ 7.	gene_phenotype
69726	2	333733	5	NULL	NULL	0	NULL	Yil113p	NucleicAcid		does not regulate					Fus3p	GP				NULL		0	NULL	NULL	NULL	gw60_febslett_527_1_186_s_190	12220658	This conclusion is supported by our own findings in which a  YIL113w disruptant strain exhibited a normal response to mating pheromone, indicating that Yil113p is not involved in regulating the Fus3p MAPK (M.C., unpublished observations) and by the results of a study in which disruption of  YIL113w alone or in combination with  PTP2 and/or  MSG5 was found to have no effect on phosphorylation of the Hog1p MAPK, indicating that Yil113p is not involved in regulating the response to osmotic stress in  S. cerevisiae [ 7.	gene_phenotype
69727	3	333733	5	NULL	NULL	0	NULL	Fus3p	GP		is a type of					MAPK	GP				NULL		0	NULL	NULL	NULL	gw60_febslett_527_1_186_s_190	12220658	This conclusion is supported by our own findings in which a  YIL113w disruptant strain exhibited a normal response to mating pheromone, indicating that Yil113p is not involved in regulating the Fus3p MAPK (M.C., unpublished observations) and by the results of a study in which disruption of  YIL113w alone or in combination with  PTP2 and/or  MSG5 was found to have no effect on phosphorylation of the Hog1p MAPK, indicating that Yil113p is not involved in regulating the response to osmotic stress in  S. cerevisiae [ 7.	gene_phenotype
69729	4	333733	5	NULL	NULL	0	NULL	YIL113w	NucleicAcid	disruption of	does not effect					Hog1p	GP	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_febslett_527_1_186_s_190	12220658	This conclusion is supported by our own findings in which a  YIL113w disruptant strain exhibited a normal response to mating pheromone, indicating that Yil113p is not involved in regulating the Fus3p MAPK (M.C., unpublished observations) and by the results of a study in which disruption of  YIL113w alone or in combination with  PTP2 and/or  MSG5 was found to have no effect on phosphorylation of the Hog1p MAPK, indicating that Yil113p is not involved in regulating the response to osmotic stress in  S. cerevisiae [ 7.	gene_phenotype
69730	5	333733	5	NULL	NULL	0	NULL	Hog1p	GP		is a type of					MAPK	GP				NULL		0	NULL	NULL	NULL	gw60_febslett_527_1_186_s_190	12220658	This conclusion is supported by our own findings in which a  YIL113w disruptant strain exhibited a normal response to mating pheromone, indicating that Yil113p is not involved in regulating the Fus3p MAPK (M.C., unpublished observations) and by the results of a study in which disruption of  YIL113w alone or in combination with  PTP2 and/or  MSG5 was found to have no effect on phosphorylation of the Hog1p MAPK, indicating that Yil113p is not involved in regulating the response to osmotic stress in  S. cerevisiae [ 7.	gene_phenotype
69731	6	333733	5	NULL	NULL	NULL	NULL	Yil113p	NucleicAcid		does not regulate					osmotic stress	PhysicalPhenomenon	response to			NULL	S. cerevisiae	NULL	NULL	NULL	NULL	gw60_febslett_527_1_186_s_190	12220658	This conclusion is supported by our own findings in which a  YIL113w disruptant strain exhibited a normal response to mating pheromone, indicating that Yil113p is not involved in regulating the Fus3p MAPK (M.C., unpublished observations) and by the results of a study in which disruption of  YIL113w alone or in combination with  PTP2 and/or  MSG5 was found to have no effect on phosphorylation of the Hog1p MAPK, indicating that Yil113p is not involved in regulating the response to osmotic stress in  S. cerevisiae [ 7.	gene_phenotype
69734	1	333734	5	NULL	NULL	0	NULL	YKL174c	NucleicAcid		encodes					TPO5 protein	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_13_12637_s_96	15668236	Inhibition of putrescine and spermidine uptake activity by TPO5 protein encoded by  YKL174c.	gene_phenotype
69735	2	333734	5	NULL	NULL	0	NULL	TPO5 protein	GP		inhibits					putrescine	Chemical	uptake of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_13_12637_s_96	15668236	Inhibition of putrescine and spermidine uptake activity by TPO5 protein encoded by  YKL174c.	gene_phenotype
69737	3	333734	5	NULL	NULL	0	NULL	TPO5 protein	GP		inhibits					spermidine	Chemical	uptake of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_13_12637_s_96	15668236	Inhibition of putrescine and spermidine uptake activity by TPO5 protein encoded by  YKL174c.	gene_phenotype
69739	1	333735	5	NULL	NULL	0	NULL	YKL174c	NucleicAcid		encodes					TPO5 protein	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_13_12637_s_111	15668236	Effect of amino acids on putrescine excretion activity by TPO5 protein encoded by  YKL174c.	gene_phenotype
69740	2	333735	5	NULL	NULL	0	NULL	TPO5 protein	GP		activates					putrescine	Chemical	excretion of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_13_12637_s_111	15668236	Effect of amino acids on putrescine excretion activity by TPO5 protein encoded by  YKL174c.	gene_phenotype
69741	3	333735	5	NULL	NULL	0	NULL	amino acids	AminoAcid		effects		possibly			statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_13_12637_s_111	15668236	Effect of amino acids on putrescine excretion activity by TPO5 protein encoded by  YKL174c.	gene_phenotype
69742	1	333736	5	NULL	NULL	0	NULL	YKL174c protein	GP		is homologous to		highly			UGA4	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_13_12637_s_76	15668236	Among these proteins, there is one, termed YKL174c, whose function is unknown but which is highly homologous with UGA4, a gamma-aminobutyric acid and putrescine transport protein on the vacuolar membrane ( ).	gene_phenotype
69744	2	333736	5	NULL	NULL	0	NULL	UGA4	GP		is present in					vacuolar membrane	CellComponent				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_13_12637_s_76	15668236	Among these proteins, there is one, termed YKL174c, whose function is unknown but which is highly homologous with UGA4, a gamma-aminobutyric acid and putrescine transport protein on the vacuolar membrane ( ).	gene_phenotype
69745	3	333736	5	NULL	NULL	0	NULL	UGA4	GP		is a type of					gamma-aminobutyric acid and putrescine transport protein	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_13_12637_s_76	15668236	Among these proteins, there is one, termed YKL174c, whose function is unknown but which is highly homologous with UGA4, a gamma-aminobutyric acid and putrescine transport protein on the vacuolar membrane ( ).	gene_phenotype
69747	1	333737	5	NULL	NULL	0	NULL	YKL174c gene	GP		is homologous to		highly			UGA4	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_13_12637_s_203	15668236	We studied the function of a protein encoded by an unidentified gene  YKL174c, which has high homology with UGA4, a member of the family of amino acid-polyamine-organocation transporters in  S. cerevisiae.	gene_phenotype
69748	2	333737	5	NULL	NULL	NULL	NULL	UGA4	GP		is a member of					amino acid-polyamine-organocation transporters family	GP				NULL	S. cerevisiae	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_13_12637_s_203	15668236	We studied the function of a protein encoded by an unidentified gene  YKL174c, which has high homology with UGA4, a member of the family of amino acid-polyamine-organocation transporters in  S. cerevisiae.	gene_phenotype
69749	1	333739	5	NULL	NULL	0	NULL	ydl117w cells	Cell		is defective in					cytokinesis	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_361	14587103	However,   ydl117w cells not only show defects in cytokinesis but also exhibit an aberrant mother-bud  neck phenotype, which often appears as a large, bent or misshapen cell (Korinek  et al., [ 2000]).	gene_phenotype
69750	2	333739	5	NULL	NULL	0	NULL	ydl117w cells	Cell		exhibit					mother-bud neck phenotype	PhysicalPhenomenon	aberrant			NULL		0	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_361	14587103	However,   ydl117w cells not only show defects in cytokinesis but also exhibit an aberrant mother-bud  neck phenotype, which often appears as a large, bent or misshapen cell (Korinek  et al., [ 2000]).	gene_phenotype
69751	3	333739	5	NULL	NULL	0	NULL	mother-bud neck phenotype	PhysicalPhenomenon	aberrant	appears as					large cell	Cell				NULL		0	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_361	14587103	However,   ydl117w cells not only show defects in cytokinesis but also exhibit an aberrant mother-bud  neck phenotype, which often appears as a large, bent or misshapen cell (Korinek  et al., [ 2000]).	gene_phenotype
69752	4	333739	5	NULL	NULL	0	NULL	mother-bud neck phenotype	PhysicalPhenomenon	aberrant	appears as					bent cell	Cell				NULL		0	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_361	14587103	However,   ydl117w cells not only show defects in cytokinesis but also exhibit an aberrant mother-bud  neck phenotype, which often appears as a large, bent or misshapen cell (Korinek  et al., [ 2000]).	gene_phenotype
69753	5	333739	5	NULL	NULL	0	NULL	mother-bud neck phenotype	PhysicalPhenomenon	aberrant	appears as					misshapen cell	Cell				NULL		0	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_361	14587103	However,   ydl117w cells not only show defects in cytokinesis but also exhibit an aberrant mother-bud  neck phenotype, which often appears as a large, bent or misshapen cell (Korinek  et al., [ 2000]).	gene_phenotype
69754	6	333739	5	NULL	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_361	14587103	However,   ydl117w cells not only show defects in cytokinesis but also exhibit an aberrant mother-bud  neck phenotype, which often appears as a large, bent or misshapen cell (Korinek  et al., [ 2000]).	gene_phenotype
69755	7	333739	5	NULL	NULL	0	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_14_1189_s_361	14587103	However,   ydl117w cells not only show defects in cytokinesis but also exhibit an aberrant mother-bud  neck phenotype, which often appears as a large, bent or misshapen cell (Korinek  et al., [ 2000]).	gene_phenotype
69756	1	333740	5	NULL	NULL	0	NULL	Ydl117w	NucleicAcid		is the locus name of					Cyk3	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_139	16498703	Ydl117w  Cyk3  1 SH3-domain protein located in the mother-bud neck and the cytokinetic actin ring;  mutant phenotype and genetic interactions suggest a role in cytokinesis  LIP  [ 20]	gene_phenotype
69757	2	333740	5	NULL	NULL	0	NULL	Cyk3	GP		is a type of					SH3-domain protein	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_139	16498703	Ydl117w  Cyk3  1 SH3-domain protein located in the mother-bud neck and the cytokinetic actin ring;  mutant phenotype and genetic interactions suggest a role in cytokinesis  LIP  [ 20]	gene_phenotype
69758	3	333740	5	NULL	NULL	0	NULL	Cyk3	GP		is located in					mother-bud neck	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_139	16498703	Ydl117w  Cyk3  1 SH3-domain protein located in the mother-bud neck and the cytokinetic actin ring;  mutant phenotype and genetic interactions suggest a role in cytokinesis  LIP  [ 20]	gene_phenotype
69759	4	333740	5	NULL	NULL	0	NULL	Cyk3	GP		is located in					cytokinetic actin ring	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_139	16498703	Ydl117w  Cyk3  1 SH3-domain protein located in the mother-bud neck and the cytokinetic actin ring;  mutant phenotype and genetic interactions suggest a role in cytokinesis  LIP  [ 20]	gene_phenotype
69760	5	333740	5	NULL	NULL	0	NULL	Cyk3	GP		plays a role in					cytokinesis	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_3_159_s_139	16498703	Ydl117w  Cyk3  1 SH3-domain protein located in the mother-bud neck and the cytokinetic actin ring;  mutant phenotype and genetic interactions suggest a role in cytokinesis  LIP  [ 20]	gene_phenotype
69761	1	333744	5	NULL	NULL	0	NULL	GST - Pus7	GP		is a type of					fusion protein	GP				NULL		0	NULL	NULL	NULL	gw60_embo_22_8_1889_s_76	12682021	Pseudouridylase activity of the GST - Pus7 (YOR243c) fusion protein expressed in either  S.cerevisiae (lanes 1 - 4) or  E.coli (lanes 5 - 8) was assayed  in vitro and compared.	gene_phenotype
69764	2	333744	5	NULL	NULL	0	NULL	YOR243c	NucleicAcid		is the locus name of					Pus7	GP				NULL		0	NULL	NULL	NULL	gw60_embo_22_8_1889_s_76	12682021	Pseudouridylase activity of the GST - Pus7 (YOR243c) fusion protein expressed in either  S.cerevisiae (lanes 1 - 4) or  E.coli (lanes 5 - 8) was assayed  in vitro and compared.	gene_phenotype
69765	3	333744	5	NULL	NULL	NULL	NULL	GST - Pus7	GP		activates					pseudouridylase	GP				NULL	S.cerevisiae, in vitro	NULL	NULL	NULL	NULL	gw60_embo_22_8_1889_s_76	12682021	Pseudouridylase activity of the GST - Pus7 (YOR243c) fusion protein expressed in either  S.cerevisiae (lanes 1 - 4) or  E.coli (lanes 5 - 8) was assayed  in vitro and compared.	gene_phenotype
69766	4	333744	5	NULL	NULL	NULL	NULL	GST - Pus7	GP		activates					pseudouridylase	GP				NULL	E.coli, in vitro	NULL	NULL	NULL	NULL	gw60_embo_22_8_1889_s_76	12682021	Pseudouridylase activity of the GST - Pus7 (YOR243c) fusion protein expressed in either  S.cerevisiae (lanes 1 - 4) or  E.coli (lanes 5 - 8) was assayed  in vitro and compared.	gene_phenotype
69769	1	333745	5	NULL	NULL	0	NULL	psi35	GP		is formed in					U2	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_embo_22_8_1889_s_7	12682021	When the GST YOR243c protein is expressed  in  Escherichia coli, pseudouridylation activity is comparable to that expressed in  S.cerevisiae, demonstrating that this protein (designated Pus7) alone can catalyze psi35 formation in U2.	gene_phenotype
69770	2	333745	5	NULL	NULL	0	NULL	Pus7 protein	GP		catalyzes					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_embo_22_8_1889_s_7	12682021	When the GST YOR243c protein is expressed  in  Escherichia coli, pseudouridylation activity is comparable to that expressed in  S.cerevisiae, demonstrating that this protein (designated Pus7) alone can catalyze psi35 formation in U2.	gene_phenotype
69771	1	333746	5	NULL	NULL	0	NULL	YOR243c protein	GP		catalyzes					U2 snRNA	NucleicAcid	yeast;;pseudouridylation		position 35	NULL		0	NULL	NULL	NULL	gw70_embo_22_8_1889_s_72	12682021	These results clearly demonstrate that YOR243c encodes a protein that catalyzes  yeast U2 snRNA pseudouridylation at position 35, and demonstrate further that the  activity occurs in a guide RNA-independent manner.	gene_phenotype
69772	2	333746	5	NULL	NULL	0	NULL	statement 1	Process		is dependent on					guide RNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_embo_22_8_1889_s_72	12682021	These results clearly demonstrate that YOR243c encodes a protein that catalyzes  yeast U2 snRNA pseudouridylation at position 35, and demonstrate further that the  activity occurs in a guide RNA-independent manner.	gene_phenotype
69773	1	333747	5	NULL	NULL	0	NULL	YOR243c	NucleicAcid		is the locus name of					Pus7	GP				NULL		0	NULL	NULL	NULL	gw70_embo_22_8_1889_s_74	12682021	Figure 3  seudouridylase activity of the GST Pus7 (YOR243c) fusion protein expressed in either   S.cerevisiae (lanes 1 4) or  E.coli (lanes 5 8) was assayed  in vitro and compared.	gene_phenotype
69774	2	333747	5	NULL	NULL	NULL	NULL	GST - Pus7	GP		activates					pseudouridylase	GP				NULL	S.cerevisiae, in vitro	NULL	NULL	NULL	NULL	gw70_embo_22_8_1889_s_74	12682021	Figure 3  seudouridylase activity of the GST Pus7 (YOR243c) fusion protein expressed in either   S.cerevisiae (lanes 1 4) or  E.coli (lanes 5 8) was assayed  in vitro and compared.	gene_phenotype
69775	3	333747	5	NULL	NULL	0	NULL	GST - Pus7	GP		activates					pseudouridylase	GP				NULL	E.coli, in vitro	0	NULL	NULL	NULL	gw70_embo_22_8_1889_s_74	12682021	Figure 3  seudouridylase activity of the GST Pus7 (YOR243c) fusion protein expressed in either   S.cerevisiae (lanes 1 4) or  E.coli (lanes 5 8) was assayed  in vitro and compared.	gene_phenotype
69776	4	333747	5	NULL	NULL	0	NULL	GST Pus7	GP		is a type of					fusion protein	GP				NULL		0	NULL	NULL	NULL	gw70_embo_22_8_1889_s_74	12682021	Figure 3  seudouridylase activity of the GST Pus7 (YOR243c) fusion protein expressed in either   S.cerevisiae (lanes 1 4) or  E.coli (lanes 5 8) was assayed  in vitro and compared.	gene_phenotype
69861	1	333748	5	NULL	NULL	0	NULL	YOR243c protein	GP		catalyzes					U2 snRNA	NucleicAcid	yeast;;pseudouridylation of		position 35	NULL		0	NULL	NULL	NULL	gw60_embo_22_8_1889_s_73	12682021	These results clearly demonstrate that YOR243c encodes a protein that catalyzes yeast U2 snRNA pseudouridylation at position 35, and demonstrate further that the activity occurs in a guide RNA-independent manner.	gene_phenotype
69862	2	333748	5	NULL	NULL	0	NULL	statement 1	Process		is dependent on					guide RNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_embo_22_8_1889_s_73	12682021	These results clearly demonstrate that YOR243c encodes a protein that catalyzes yeast U2 snRNA pseudouridylation at position 35, and demonstrate further that the activity occurs in a guide RNA-independent manner.	gene_phenotype
69863	1	333750	5	NULL	NULL	0	NULL	Ygr223c	NucleicAcid		has no function in		obvious			Cvt pathway	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_36_37741_s_127	15194695	Ygr223c has no obvious function in the Cvt pathway and autophagy.	gene_phenotype
69864	2	333750	5	NULL	NULL	0	NULL	Ygr223c	NucleicAcid		has no function in		obvious			autophagy	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_36_37741_s_127	15194695	Ygr223c has no obvious function in the Cvt pathway and autophagy.	gene_phenotype
69865	1	333752	5	NULL	NULL	0	NULL	Atg18	GP		is required for					autophagy	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_8_3553_s_314	15155809	Atg18 is required for all types of autophagy, whereas a strong phenotype has not yet been found for Ygr223c.	gene_phenotype
69866	2	333752	5	NULL	NULL	0	NULL	Ygr223c	NucleicAcid		does not show					phenotype	PhysicalPhenomenon	strong			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_8_3553_s_314	15155809	Atg18 is required for all types of autophagy, whereas a strong phenotype has not yet been found for Ygr223c.	gene_phenotype
69867	1	333753	5	NULL	NULL	NULL	NULL	Atg18 protein	GP	yeast	is homologous to					Atg21 protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_36_37741_s_122	15194695	The Homologous Proteins Atg18 and Atg21 Play Distinct Roles in Autophagy and the Cvt Pathway -- Atg21 has two yeast homologues, Atg18 ( 20% identity) and the protein of so far unknown function, Ygr223c ( 14% identity).	gene_phenotype
69868	2	333753	5	NULL	NULL	0	NULL	Atg18 protein	GP		plays a role in		distinct			autophagy	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_36_37741_s_122	15194695	The Homologous Proteins Atg18 and Atg21 Play Distinct Roles in Autophagy and the Cvt Pathway -- Atg21 has two yeast homologues, Atg18 ( 20% identity) and the protein of so far unknown function, Ygr223c ( 14% identity).	gene_phenotype
69869	3	333753	5	NULL	NULL	0	NULL	Atg18 protein	GP		plays a role in		distinct			Cvt Pathway	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_36_37741_s_122	15194695	The Homologous Proteins Atg18 and Atg21 Play Distinct Roles in Autophagy and the Cvt Pathway -- Atg21 has two yeast homologues, Atg18 ( 20% identity) and the protein of so far unknown function, Ygr223c ( 14% identity).	gene_phenotype
69870	4	333753	5	NULL	NULL	0	NULL	Atg21 protein	GP		plays a role in		distinct			autophagy	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_36_37741_s_122	15194695	The Homologous Proteins Atg18 and Atg21 Play Distinct Roles in Autophagy and the Cvt Pathway -- Atg21 has two yeast homologues, Atg18 ( 20% identity) and the protein of so far unknown function, Ygr223c ( 14% identity).	gene_phenotype
69871	5	333753	5	NULL	NULL	0	NULL	Atg21 protein	GP		plays a role in		distinct			Cvt Pathway	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_36_37741_s_122	15194695	The Homologous Proteins Atg18 and Atg21 Play Distinct Roles in Autophagy and the Cvt Pathway -- Atg21 has two yeast homologues, Atg18 ( 20% identity) and the protein of so far unknown function, Ygr223c ( 14% identity).	gene_phenotype
69872	6	333753	5	NULL	NULL	0	NULL	Atg21 protein	GP		is homologous to					Ygr223c protein	GP	yeast			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_36_37741_s_122	15194695	The Homologous Proteins Atg18 and Atg21 Play Distinct Roles in Autophagy and the Cvt Pathway -- Atg21 has two yeast homologues, Atg18 ( 20% identity) and the protein of so far unknown function, Ygr223c ( 14% identity).	gene_phenotype
69873	1	333754	5	NULL	NULL	0	NULL	Atg21	GP		is homologous to					Atg21 protein	GP	yeast			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_36_37741_s_345	15194695	Atg21 is a very promising candidate for studies aiming to learn more about the mechanistic features and differences of autophagy and the Cvt pathway, since it shares homologies with two further yeast proteins, Atg18 and Ygr223c.	gene_phenotype
69874	2	333754	5	NULL	NULL	0	NULL	Atg21	GP		is homologous to					Ygr223c protein	GP	yeast			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_36_37741_s_345	15194695	Atg21 is a very promising candidate for studies aiming to learn more about the mechanistic features and differences of autophagy and the Cvt pathway, since it shares homologies with two further yeast proteins, Atg18 and Ygr223c.	gene_phenotype
69875	3	333754	5	NULL	NULL	0	NULL	Atg21	GP		plays a role in		possibly			autophagy	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_36_37741_s_345	15194695	Atg21 is a very promising candidate for studies aiming to learn more about the mechanistic features and differences of autophagy and the Cvt pathway, since it shares homologies with two further yeast proteins, Atg18 and Ygr223c.	gene_phenotype
69876	4	333754	5	NULL	NULL	0	NULL	Atg21	GP		plays a role in		possibly			Cvt pathway	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_36_37741_s_345	15194695	Atg21 is a very promising candidate for studies aiming to learn more about the mechanistic features and differences of autophagy and the Cvt pathway, since it shares homologies with two further yeast proteins, Atg18 and Ygr223c.	gene_phenotype
69877	1	333755	5	NULL	NULL	0	NULL	Ygr223c	NucleicAcid		has no function in		obvious			Cvt pathway	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_36_37741_s_346	15194695	As shown here, Ygr223c has no obvious function in the Cvt pathway or autophagy ( Fig. 1 A), whereas Atg18 has been shown to function in both biogenesis of autophagosomes and Cvt vesicles ( ,  ).	gene_phenotype
69878	2	333755	5	NULL	NULL	0	NULL	Ygr223c	NucleicAcid		has no function in		obvious			autophagy	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_36_37741_s_346	15194695	As shown here, Ygr223c has no obvious function in the Cvt pathway or autophagy ( Fig. 1 A), whereas Atg18 has been shown to function in both biogenesis of autophagosomes and Cvt vesicles ( ,  ).	gene_phenotype
69879	3	333755	5	NULL	NULL	0	NULL	Atg18	GP		functions in					autophagosomes	CellComponent	biogenesis of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_36_37741_s_346	15194695	As shown here, Ygr223c has no obvious function in the Cvt pathway or autophagy ( Fig. 1 A), whereas Atg18 has been shown to function in both biogenesis of autophagosomes and Cvt vesicles ( ,  ).	gene_phenotype
69880	4	333755	5	NULL	NULL	0	NULL	Atg18	GP		functions in					Cvt vesicles	CellComponent	biogenesis of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_36_37741_s_346	15194695	As shown here, Ygr223c has no obvious function in the Cvt pathway or autophagy ( Fig. 1 A), whereas Atg18 has been shown to function in both biogenesis of autophagosomes and Cvt vesicles ( ,  ).	gene_phenotype
69881	1	333756	5	NULL	NULL	NULL	NULL	Atg8	GP		is localized to		efficiently			PAS	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_8_3553_s_196	15155809	Atg21 Is Required for Efficient Localization of Atg8 to the PAS   As mentioned above, no Cvt pathway- or autophagy-specific proteins were found to be required for the localization of Atg21, and the Atg18, Atg21, and Ygr223c proteins were not dependent on each other for localization (our unpublished data).	gene_phenotype
69882	2	333756	5	NULL	NULL	0	NULL	Atg21	GP		is required for					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_8_3553_s_196	15155809	Atg21 Is Required for Efficient Localization of Atg8 to the PAS   As mentioned above, no Cvt pathway- or autophagy-specific proteins were found to be required for the localization of Atg21, and the Atg18, Atg21, and Ygr223c proteins were not dependent on each other for localization (our unpublished data).	gene_phenotype
69883	3	333756	5	NULL	NULL	0	NULL	Cvt pathway proteins	GP		is not required for					Atg21	GP	localization of			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_8_3553_s_196	15155809	Atg21 Is Required for Efficient Localization of Atg8 to the PAS   As mentioned above, no Cvt pathway- or autophagy-specific proteins were found to be required for the localization of Atg21, and the Atg18, Atg21, and Ygr223c proteins were not dependent on each other for localization (our unpublished data).	gene_phenotype
69884	4	333756	5	NULL	NULL	0	NULL	autophagy-specific proteins	GP		is not required for					Atg21	GP	localization of			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_8_3553_s_196	15155809	Atg21 Is Required for Efficient Localization of Atg8 to the PAS   As mentioned above, no Cvt pathway- or autophagy-specific proteins were found to be required for the localization of Atg21, and the Atg18, Atg21, and Ygr223c proteins were not dependent on each other for localization (our unpublished data).	gene_phenotype
69885	5	333756	5	NULL	NULL	0	NULL	Atg18 protein	GP	localization of	is not dependent on					Atg21 protein	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_8_3553_s_196	15155809	Atg21 Is Required for Efficient Localization of Atg8 to the PAS   As mentioned above, no Cvt pathway- or autophagy-specific proteins were found to be required for the localization of Atg21, and the Atg18, Atg21, and Ygr223c proteins were not dependent on each other for localization (our unpublished data).	gene_phenotype
69886	6	333756	5	NULL	NULL	0	NULL	Atg21 protein	GP	localization of	is not dependent on					Ygr223c protein	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_8_3553_s_196	15155809	Atg21 Is Required for Efficient Localization of Atg8 to the PAS   As mentioned above, no Cvt pathway- or autophagy-specific proteins were found to be required for the localization of Atg21, and the Atg18, Atg21, and Ygr223c proteins were not dependent on each other for localization (our unpublished data).	gene_phenotype
69887	7	333756	5	NULL	NULL	0	NULL	Atg21 protein	GP	localization of	is not dependent on					Ygr223c protein	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_8_3553_s_196	15155809	Atg21 Is Required for Efficient Localization of Atg8 to the PAS   As mentioned above, no Cvt pathway- or autophagy-specific proteins were found to be required for the localization of Atg21, and the Atg18, Atg21, and Ygr223c proteins were not dependent on each other for localization (our unpublished data).	gene_phenotype
69888	8	333756	5	NULL	NULL	0	NULL	Atg21 protein	GP	localization of	is not dependent on					Atg18 protein	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_8_3553_s_196	15155809	Atg21 Is Required for Efficient Localization of Atg8 to the PAS   As mentioned above, no Cvt pathway- or autophagy-specific proteins were found to be required for the localization of Atg21, and the Atg18, Atg21, and Ygr223c proteins were not dependent on each other for localization (our unpublished data).	gene_phenotype
69889	9	333756	5	NULL	NULL	0	NULL	Ygr223c protein	GP	localization of	is not dependent on					Atg21 protein	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_8_3553_s_196	15155809	Atg21 Is Required for Efficient Localization of Atg8 to the PAS   As mentioned above, no Cvt pathway- or autophagy-specific proteins were found to be required for the localization of Atg21, and the Atg18, Atg21, and Ygr223c proteins were not dependent on each other for localization (our unpublished data).	gene_phenotype
69890	10	333756	5	NULL	NULL	0	NULL	Ygr223c protein	GP	localization of	is not dependent on					Atg18 protein	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_8_3553_s_196	15155809	Atg21 Is Required for Efficient Localization of Atg8 to the PAS   As mentioned above, no Cvt pathway- or autophagy-specific proteins were found to be required for the localization of Atg21, and the Atg18, Atg21, and Ygr223c proteins were not dependent on each other for localization (our unpublished data).	gene_phenotype
69891	1	333759	5	NULL	NULL	0	NULL	Af1521	GP		is homologous to			macro domain		YBR022W gene product	GP	yeast			NULL		0	NULL	NULL	NULL	gw70_embo_24_11_1911_s_48	15902274	A screen in the yeast  Saccharomyces cerevisiae identified a protein with homology to the  macro domain of Af1521, the YBR022W gene product, as exhibiting ADP-ribose-1"`-phosphate  (Appr-1"`-P) processing activity (  et al).	gene_phenotype
69892	2	333759	5	NULL	NULL	0	NULL	YBR022W gene product	GP		activates					ADP-ribose-1"`-phosphate (Appr-1"`-P)	Chemical	processing of			NULL		0	NULL	NULL	NULL	gw70_embo_24_11_1911_s_48	15902274	A screen in the yeast  Saccharomyces cerevisiae identified a protein with homology to the  macro domain of Af1521, the YBR022W gene product, as exhibiting ADP-ribose-1"`-phosphate  (Appr-1"`-P) processing activity (  et al).	gene_phenotype
69903	1	333762	5	NULL	NULL	0	NULL	YGR173w	NucleicAcid		plays a role in		potentially			purine salvage	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_7_553_s_408	16710832	For YGR173w, weak evidence was found for the present annotation  purine salvage, tRNA modification and ribonucleoside monophosphate biosynthesis pathways  and GeneFAS annotated similar terms (cell growth and/or maintenance, metabolism,  cell organization and biogenesis nucleobase, nucleoside, nucleotide and nucleic acid  metabolism, cytoplasm organization and biogenesis, transport, ribosome biogenesis  and assembly, transcription, RNA metabolism biosynthesis transcription, DNA-dependent  ribosome biogenesis, RNA processing, organic acid metabolism, carbohydrate metabolism,  aromatic compound metabolism, heterocycle metabolism, ion transport, catabolism).	gene_phenotype
69904	2	333762	5	NULL	NULL	0	NULL	YGR173w	NucleicAcid		plays a role in		potentially			tRNA	NucleicAcid	modification of			NULL		0	NULL	NULL	NULL	gw70_yeast_23_7_553_s_408	16710832	For YGR173w, weak evidence was found for the present annotation  purine salvage, tRNA modification and ribonucleoside monophosphate biosynthesis pathways  and GeneFAS annotated similar terms (cell growth and/or maintenance, metabolism,  cell organization and biogenesis nucleobase, nucleoside, nucleotide and nucleic acid  metabolism, cytoplasm organization and biogenesis, transport, ribosome biogenesis  and assembly, transcription, RNA metabolism biosynthesis transcription, DNA-dependent  ribosome biogenesis, RNA processing, organic acid metabolism, carbohydrate metabolism,  aromatic compound metabolism, heterocycle metabolism, ion transport, catabolism).	gene_phenotype
69905	3	333762	5	NULL	NULL	0	NULL	YGR173w	NucleicAcid		plays a role in		potentially			ribonucleoside monophosphate biosynthesis pathways	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_7_553_s_408	16710832	For YGR173w, weak evidence was found for the present annotation  purine salvage, tRNA modification and ribonucleoside monophosphate biosynthesis pathways  and GeneFAS annotated similar terms (cell growth and/or maintenance, metabolism,  cell organization and biogenesis nucleobase, nucleoside, nucleotide and nucleic acid  metabolism, cytoplasm organization and biogenesis, transport, ribosome biogenesis  and assembly, transcription, RNA metabolism biosynthesis transcription, DNA-dependent  ribosome biogenesis, RNA processing, organic acid metabolism, carbohydrate metabolism,  aromatic compound metabolism, heterocycle metabolism, ion transport, catabolism).	gene_phenotype
69908	1	333763	5	NULL	NULL	0	NULL	YPR016c	NucleicAcid		is required for					viability	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_17_11653_s_136	10206977	None of the viable segregants were TRP+, indicating that  YPR016c is required for viability.	gene_phenotype
69909	1	333764	5	NULL	NULL	NULL	NULL	YPR016c gene product 	GP	yeast	is a synonym of					eIF6	GP	yeast			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_17_11653_s_25	10206977	Furthermore, expression of either  YPR016c-GFP or murine eIF6-GFP fusion proteins restored viability, suggesting that the  YPR016c gene product is indeed yeast eIF6.	gene_phenotype
69910	2	333764	5	NULL	NULL	0	NULL	YPR016c-GFP	GP	expression of	restores					viability	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_17_11653_s_25	10206977	Furthermore, expression of either  YPR016c-GFP or murine eIF6-GFP fusion proteins restored viability, suggesting that the  YPR016c gene product is indeed yeast eIF6.	gene_phenotype
69911	3	333764	5	NULL	NULL	0	NULL	eIF6-GFP	GP	murine;;expression of	restores					viability	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_17_11653_s_25	10206977	Furthermore, expression of either  YPR016c-GFP or murine eIF6-GFP fusion proteins restored viability, suggesting that the  YPR016c gene product is indeed yeast eIF6.	gene_phenotype
69912	4	333764	5	NULL	NULL	0	NULL	eIF6-GFP	GP		is a type of					fusion protein	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_17_11653_s_25	10206977	Furthermore, expression of either  YPR016c-GFP or murine eIF6-GFP fusion proteins restored viability, suggesting that the  YPR016c gene product is indeed yeast eIF6.	gene_phenotype
69913	5	333764	5	NULL	NULL	0	NULL	YPR016c-GFP	GP		is a type of					fusion protein	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_17_11653_s_25	10206977	Furthermore, expression of either  YPR016c-GFP or murine eIF6-GFP fusion proteins restored viability, suggesting that the  YPR016c gene product is indeed yeast eIF6.	gene_phenotype
69915	1	333766	5	NULL	NULL	0	NULL	YPR016c-GFP	GP		substitute for					YPR016c protein product	GP	endogenous			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_17_11653_s_140	10206977	Tetrad analysis of LWY1 harboring pLW-2 produced four viable segregants (two TRP+ segregants and two TRP  segregants), indicating that the  YPR016c-GFP fusion protein was functional and could substitute for the endogenous  YPR016c protein product.	gene_phenotype
69916	2	333766	5	NULL	NULL	0	NULL	YPR016c-GFP	GP		is a type of					fusion protein	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_17_11653_s_140	10206977	Tetrad analysis of LWY1 harboring pLW-2 produced four viable segregants (two TRP+ segregants and two TRP  segregants), indicating that the  YPR016c-GFP fusion protein was functional and could substitute for the endogenous  YPR016c protein product.	gene_phenotype
69918	1	333767	5	NULL	NULL	0	NULL	YPR016c	GP	presence of	restores					viability	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_17_11653_s_7	10206977	Viability was restored in the presence of either  YPR016c or murine eIF6, when either was expressed as amino-terminal green fluorescent protein fusion protein.	gene_phenotype
69920	2	333767	5	NULL	NULL	0	NULL	eIF6	GP	presence of;;murine	restores					viability	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_17_11653_s_7	10206977	Viability was restored in the presence of either  YPR016c or murine eIF6, when either was expressed as amino-terminal green fluorescent protein fusion protein.	gene_phenotype
69922	3	333767	5	NULL	NULL	0	NULL	eIF6	GP	murine	is expressed as			amino-terminal		green fluorescent protein fusion protein	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_17_11653_s_7	10206977	Viability was restored in the presence of either  YPR016c or murine eIF6, when either was expressed as amino-terminal green fluorescent protein fusion protein.	gene_phenotype
69923	4	333767	5	NULL	NULL	0	NULL	YPR016c	GP		is expressed as			amino-terminal		green fluorescent protein fusion protein	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_17_11653_s_7	10206977	Viability was restored in the presence of either  YPR016c or murine eIF6, when either was expressed as amino-terminal green fluorescent protein fusion protein.	gene_phenotype
69924	1	333768	5	NULL	NULL	NULL	NULL	eIF6	GP		is homologous to					TIF6	GP	yeast			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_5_1453_s_15	11238882	Detailed characterization of the yeast gene encoding eIF6, designated  TIF6, showed that  TIF6 is a single-copy gene that maps on chromosome XVI (as YPR016C) and is essential for cell growth and viability.	gene_phenotype
69926	2	333768	5	NULL	NULL	NULL	NULL	TIF6	GP	yeast	is a type of					single-copy gene	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_5_1453_s_15	11238882	Detailed characterization of the yeast gene encoding eIF6, designated  TIF6, showed that  TIF6 is a single-copy gene that maps on chromosome XVI (as YPR016C) and is essential for cell growth and viability.	gene_phenotype
69927	3	333768	5	NULL	NULL	NULL	NULL	TIF6 gene	GP	yeast	maps to					chromosome XVI	Chromosome				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_5_1453_s_15	11238882	Detailed characterization of the yeast gene encoding eIF6, designated  TIF6, showed that  TIF6 is a single-copy gene that maps on chromosome XVI (as YPR016C) and is essential for cell growth and viability.	gene_phenotype
69929	4	333768	5	NULL	NULL	NULL	NULL	YPR016C	NucleicAcid		is the locus name of					TIF6	GP	yeast			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_5_1453_s_15	11238882	Detailed characterization of the yeast gene encoding eIF6, designated  TIF6, showed that  TIF6 is a single-copy gene that maps on chromosome XVI (as YPR016C) and is essential for cell growth and viability.	gene_phenotype
69930	5	333768	5	NULL	NULL	NULL	NULL	TIF6	GP	yeast	is essential for					cell growth	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_5_1453_s_15	11238882	Detailed characterization of the yeast gene encoding eIF6, designated  TIF6, showed that  TIF6 is a single-copy gene that maps on chromosome XVI (as YPR016C) and is essential for cell growth and viability.	gene_phenotype
69931	6	333768	5	NULL	NULL	0	NULL	TIF6	GP	yeast	is essential for					cell viability	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_5_1453_s_15	11238882	Detailed characterization of the yeast gene encoding eIF6, designated  TIF6, showed that  TIF6 is a single-copy gene that maps on chromosome XVI (as YPR016C) and is essential for cell growth and viability.	gene_phenotype
69933	1	333769	5	NULL	NULL	0	NULL	YPR016c-GFP	GP		is a type of					fusion protein	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_17_11653_s_147	10206977	This result demonstrated that the cells were dependent upon  GAL1-regulated expression of either the  YPR016c-GFP (in LWY4) or the murine eIF6-GFP (in LWY6) fusion proteins for viability.	gene_phenotype
69934	2	333769	5	NULL	NULL	0	NULL	eIF6-GFP	GP	murine	is a type of					fusion protein	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_17_11653_s_147	10206977	This result demonstrated that the cells were dependent upon  GAL1-regulated expression of either the  YPR016c-GFP (in LWY4) or the murine eIF6-GFP (in LWY6) fusion proteins for viability.	gene_phenotype
69935	3	333769	5	NULL	NULL	0	NULL	YPR016c-GFP	GP		plays a role in					cell viability	Process				NULL	LWY4	0	NULL	NULL	NULL	gw60_jbiolchem_274_17_11653_s_147	10206977	This result demonstrated that the cells were dependent upon  GAL1-regulated expression of either the  YPR016c-GFP (in LWY4) or the murine eIF6-GFP (in LWY6) fusion proteins for viability.	gene_phenotype
69936	4	333769	5	NULL	NULL	NULL	NULL	eIF6-GFP	GP	murine	plays a role in					cell viability	Process				NULL	LWY6	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_17_11653_s_147	10206977	This result demonstrated that the cells were dependent upon  GAL1-regulated expression of either the  YPR016c-GFP (in LWY4) or the murine eIF6-GFP (in LWY6) fusion proteins for viability.	gene_phenotype
69937	1	333771	5	NULL	NULL	0	NULL	eIF6-GFP	GP	overexpression of	does not effect		major			cell growth	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_17_11653_s_143	10206977	As shown in Fig.  3 ( left side), the growth rates of LWY4 (harboring  GAL1- YPR016c-GFP) and LWY6 (harboring  GAL1-murine eIF6-GFP)  versus control appeared somewhat slower on SGal, indicating that overexpression of the eIF6-GFP fusion proteins had no major effects on cell growth.	gene_phenotype
69938	2	333771	5	NULL	NULL	0	NULL	eIF6-GFP	GP		is a type of					fusion protein	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_17_11653_s_143	10206977	As shown in Fig.  3 ( left side), the growth rates of LWY4 (harboring  GAL1- YPR016c-GFP) and LWY6 (harboring  GAL1-murine eIF6-GFP)  versus control appeared somewhat slower on SGal, indicating that overexpression of the eIF6-GFP fusion proteins had no major effects on cell growth.	gene_phenotype
69939	1	333773	5	NULL	NULL	0	NULL	autophagy mutants	GP		is sensitive to					nitrogen	Chemical				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_69_0_303_s_259	10966461	In addition,  cvt3 does not display the degree of nitrogen sensitivity typical of autophagy mutants  ( 16).	gene_phenotype
69940	2	333773	5	NULL	NULL	NULL	NULL	cvt3	GP		is sensitive to					nitrogen	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_69_0_303_s_259	10966461	In addition,  cvt3 does not display the degree of nitrogen sensitivity typical of autophagy mutants  ( 16).	gene_phenotype
69941	3	333773	5	NULL	NULL	0	NULL	statement 2	Process	degree of	lesser than					statement 1	Process	degree of			NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_69_0_303_s_259	10966461	In addition,  cvt3 does not display the degree of nitrogen sensitivity typical of autophagy mutants  ( 16).	gene_phenotype
69942	1	333774	5	NULL	NULL	0	NULL	cvt9	GP	mutant	is required for					Cvt	GP	trafficking of			NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_65_3_463_s_235	11528006	The  cvt9 mutant and the as yet uncharacterized  cvt3 mutant are the two original mutations that were identified as being required for Cvt trafficking but not for autophagy ( ).	gene_phenotype
69943	2	333774	5	NULL	NULL	0	NULL	cvt3	GP	mutant	is required for					Cvt	GP	trafficking of			NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_65_3_463_s_235	11528006	The  cvt9 mutant and the as yet uncharacterized  cvt3 mutant are the two original mutations that were identified as being required for Cvt trafficking but not for autophagy ( ).	gene_phenotype
69944	3	333774	5	NULL	NULL	0	NULL	cvt9	GP	mutant	is not required for					autophagy	Process				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_65_3_463_s_235	11528006	The  cvt9 mutant and the as yet uncharacterized  cvt3 mutant are the two original mutations that were identified as being required for Cvt trafficking but not for autophagy ( ).	gene_phenotype
69945	4	333774	5	NULL	NULL	0	NULL	cvt3	GP	mutant	is not required for					autophagy	Process				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_65_3_463_s_235	11528006	The  cvt9 mutant and the as yet uncharacterized  cvt3 mutant are the two original mutations that were identified as being required for Cvt trafficking but not for autophagy ( ).	gene_phenotype
69946	1	333775	5	NULL	NULL	0	NULL	cvt3	GP	mutant	induce					autophagy	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_139_7_1687_s_177	9412464	Induction of autophagy may be  slower in the  cvt3 mutant compared to wild-type, and the  resulting autophagosomes appear to be slightly aberrant.	gene_phenotype
69947	2	333775	5	NULL	NULL	0	NULL	Cvt	GP	wild-type	induce					autophagy	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_139_7_1687_s_177	9412464	Induction of autophagy may be  slower in the  cvt3 mutant compared to wild-type, and the  resulting autophagosomes appear to be slightly aberrant.	gene_phenotype
69948	3	333775	5	NULL	NULL	0	NULL	statement 1	Process		slower than					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_139_7_1687_s_177	9412464	Induction of autophagy may be  slower in the  cvt3 mutant compared to wild-type, and the  resulting autophagosomes appear to be slightly aberrant.	gene_phenotype
69949	4	333775	5	NULL	NULL	0	NULL	statement 1	Process		leads to					autophagosomes	CellComponent	formation of;;aberrent			NULL		0	NULL	NULL	NULL	gw60_cellbiol_139_7_1687_s_177	9412464	Induction of autophagy may be  slower in the  cvt3 mutant compared to wild-type, and the  resulting autophagosomes appear to be slightly aberrant.	gene_phenotype
70031	1	333776	5	NULL	NULL	0	NULL	cvt3	GP		is sensitive to					nitrogen	Chemical				NULL		0	NULL	NULL	NULL	gw60_annrevbiochem_69_0_303_s_212	10966461	In addition,   cvt3  does not display the degree of nitrogen sensitivity typical of  autophagy mutants ( 16).	gene_phenotype
70032	1	333777	5	NULL	NULL	0	NULL	Aut7p	GP		is stabilized in					cvt3 strain	Cell				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_8_5845_s_209	10681575	Further, Aut7p was also observed to be stabilized in the  cvt3 strain under vegetative growth conditions (data not shown).	gene_phenotype
70033	2	333777	5	NULL	NULL	0	NULL	statement 1	Process		under condition of					vegetative growth	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_8_5845_s_209	10681575	Further, Aut7p was also observed to be stabilized in the  cvt3 strain under vegetative growth conditions (data not shown).	gene_phenotype
70034	1	333778	5	NULL	NULL	0	NULL	cvt3	GP	mutant	is defective in					Cvt pathway	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_8_5845_s_220	10681575	The  cvt3 mutant is defective in the Cvt pathway but displays an essentially normal phenotype for autophagy ( 9,  10).	gene_phenotype
70035	2	333778	5	NULL	NULL	0	NULL	cvt3	GP	mutant	displays					autophagy	Process	normal phenotype for			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_8_5845_s_220	10681575	The  cvt3 mutant is defective in the Cvt pathway but displays an essentially normal phenotype for autophagy ( 9,  10).	gene_phenotype
70036	1	333779	5	NULL	NULL	0	NULL	cvt3	GP		is defective in					autophagy	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_30_17621_s_93	8663607	Three groups,  cvt3,  6, and  9, appeared less defective in autophagy than the  aut mutants using this test.	gene_phenotype
70037	2	333779	5	NULL	NULL	0	NULL	cvt6	GP		is defective in					autophagy	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_30_17621_s_93	8663607	Three groups,  cvt3,  6, and  9, appeared less defective in autophagy than the  aut mutants using this test.	gene_phenotype
70038	3	333779	5	NULL	NULL	0	NULL	cvt9	GP		is defective in					autophagy	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_30_17621_s_93	8663607	Three groups,  cvt3,  6, and  9, appeared less defective in autophagy than the  aut mutants using this test.	gene_phenotype
70039	4	333779	5	NULL	NULL	0	NULL	aut	GP	mutant	is defective in					autophagy	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_30_17621_s_93	8663607	Three groups,  cvt3,  6, and  9, appeared less defective in autophagy than the  aut mutants using this test.	gene_phenotype
70040	5	333779	5	NULL	NULL	0	NULL	statement 1	Process		lesser than					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_30_17621_s_93	8663607	Three groups,  cvt3,  6, and  9, appeared less defective in autophagy than the  aut mutants using this test.	gene_phenotype
70041	6	333779	5	NULL	NULL	0	NULL	statement 2	Process		lesser than					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_30_17621_s_93	8663607	Three groups,  cvt3,  6, and  9, appeared less defective in autophagy than the  aut mutants using this test.	gene_phenotype
70042	7	333779	5	NULL	NULL	0	NULL	statement 3	Process		lesser than					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_30_17621_s_93	8663607	Three groups,  cvt3,  6, and  9, appeared less defective in autophagy than the  aut mutants using this test.	gene_phenotype
70043	1	333782	5	NULL	NULL	0	NULL	cvt3	GP	mutant	is defective in					Cvt pathway	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_139_7_1687_s_182	9412464	The finding that  the  cvt3 mutant is defective for the Cvt pathway but not  autophagy provides independent support for the idea that  two separate but related pathways are responsible for targeting API to the vacuole.	gene_phenotype
70044	2	333782	5	NULL	NULL	0	NULL	cvt3	GP	mutant	is not defective in					autophagy	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_139_7_1687_s_182	9412464	The finding that  the  cvt3 mutant is defective for the Cvt pathway but not  autophagy provides independent support for the idea that  two separate but related pathways are responsible for targeting API to the vacuole.	gene_phenotype
70045	3	333782	5	NULL	NULL	0	NULL	API	GP		targeted to					vacuole	CellComponent				NULL		0	NULL	NULL	NULL	gw60_cellbiol_139_7_1687_s_182	9412464	The finding that  the  cvt3 mutant is defective for the Cvt pathway but not  autophagy provides independent support for the idea that  two separate but related pathways are responsible for targeting API to the vacuole.	gene_phenotype
70046	1	333784	5	NULL	NULL	0	NULL	CVT3 gene product	GP		is essential for					Cvt pathway	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_139_7_1687_s_178	9412464	These results support our biochemical analysis and suggest  that the  CVT3 gene encodes a molecule that is essential  for the Cvt pathway but not for autophagy; under starvation conditions, API can be transported by autophagy,  even though the Cvt pathway is defective.	gene_phenotype
70047	2	333784	5	NULL	NULL	0	NULL	CVT3 gene product	GP		is not essential for					autophagy	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_139_7_1687_s_178	9412464	These results support our biochemical analysis and suggest  that the  CVT3 gene encodes a molecule that is essential  for the Cvt pathway but not for autophagy; under starvation conditions, API can be transported by autophagy,  even though the Cvt pathway is defective.	gene_phenotype
70048	3	333784	5	NULL	NULL	0	NULL	API	GP		is transfered by					autophagy	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_139_7_1687_s_178	9412464	These results support our biochemical analysis and suggest  that the  CVT3 gene encodes a molecule that is essential  for the Cvt pathway but not for autophagy; under starvation conditions, API can be transported by autophagy,  even though the Cvt pathway is defective.	gene_phenotype
70049	4	333784	5	NULL	NULL	NULL	NULL	statement 3	Process		under condition of					starvation	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_139_7_1687_s_178	9412464	These results support our biochemical analysis and suggest  that the  CVT3 gene encodes a molecule that is essential  for the Cvt pathway but not for autophagy; under starvation conditions, API can be transported by autophagy,  even though the Cvt pathway is defective.	gene_phenotype
70050	5	333784	5	NULL	NULL	0	NULL	statement 3	Process		in the presence of					Cvt pathway	Process	defective			NULL		0	NULL	NULL	NULL	gw60_cellbiol_139_7_1687_s_178	9412464	These results support our biochemical analysis and suggest  that the  CVT3 gene encodes a molecule that is essential  for the Cvt pathway but not for autophagy; under starvation conditions, API can be transported by autophagy,  even though the Cvt pathway is defective.	gene_phenotype
70082	1	333785	5	NULL	NULL	0	NULL	API	GP		is transported		completely			cvt3	Cell				NULL		0	NULL	NULL	NULL	gw60_cellbiol_139_7_1687_s_180	9412464	In addition, the observation that the transport of API approaches completion  in  cvt3 under starvation conditions suggests that a selective  autophagic mechanism is used; nonselective transport of  cytosolic protein such as Pho8delta60p by autophagy appears  to plateau at ~30% import (Scott et al., 1996  ).	gene_phenotype
70083	2	333785	5	NULL	NULL	0	NULL	statement 1	Process		under condition of					starvation	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_139_7_1687_s_180	9412464	In addition, the observation that the transport of API approaches completion  in  cvt3 under starvation conditions suggests that a selective  autophagic mechanism is used; nonselective transport of  cytosolic protein such as Pho8delta60p by autophagy appears  to plateau at ~30% import (Scott et al., 1996  ).	gene_phenotype
70084	3	333785	5	NULL	NULL	0	NULL	statement 1	Process		involves					autophagic mechanism	Process	selective			NULL		0	NULL	NULL	NULL	gw60_cellbiol_139_7_1687_s_180	9412464	In addition, the observation that the transport of API approaches completion  in  cvt3 under starvation conditions suggests that a selective  autophagic mechanism is used; nonselective transport of  cytosolic protein such as Pho8delta60p by autophagy appears  to plateau at ~30% import (Scott et al., 1996  ).	gene_phenotype
70085	4	333785	5	NULL	NULL	0	NULL	Pho8delta60p	GP	nonselective;;transport of	occurs by					autophagy	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_139_7_1687_s_180	9412464	In addition, the observation that the transport of API approaches completion  in  cvt3 under starvation conditions suggests that a selective  autophagic mechanism is used; nonselective transport of  cytosolic protein such as Pho8delta60p by autophagy appears  to plateau at ~30% import (Scott et al., 1996  ).	gene_phenotype
70086	5	333785	5	NULL	NULL	0	NULL	Pho8delta60p	GP		is a type of					cytosolic protein	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_139_7_1687_s_180	9412464	In addition, the observation that the transport of API approaches completion  in  cvt3 under starvation conditions suggests that a selective  autophagic mechanism is used; nonselective transport of  cytosolic protein such as Pho8delta60p by autophagy appears  to plateau at ~30% import (Scott et al., 1996  ).	gene_phenotype
70087	1	333787	5	NULL	NULL	0	NULL	galactolipid	Chemical	defeciency	impede					node of Ranvier	CellComponent	maintenance of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_156_3_567_s_135	11827985	Galactolipid and MAG deficiencies impede node of Ranvier maintanence, not formation   The dramatic consequences of galactolipid and MAG elimination on nodal regions were observed around the life expectancy endpoint for this mutant line.	gene_phenotype
70088	2	333787	5	NULL	NULL	0	NULL	MAG	Chemical	defeciency	impede					node of Ranvier	CellComponent	maintenance of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_156_3_567_s_135	11827985	Galactolipid and MAG deficiencies impede node of Ranvier maintanence, not formation   The dramatic consequences of galactolipid and MAG elimination on nodal regions were observed around the life expectancy endpoint for this mutant line.	gene_phenotype
70089	3	333787	5	NULL	NULL	0	NULL	galactolipid	Chemical	defeciency	does not impede					node of Ranvier	CellComponent	formation of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_156_3_567_s_135	11827985	Galactolipid and MAG deficiencies impede node of Ranvier maintanence, not formation   The dramatic consequences of galactolipid and MAG elimination on nodal regions were observed around the life expectancy endpoint for this mutant line.	gene_phenotype
70090	4	333787	5	NULL	NULL	0	NULL	MAG	Chemical	defeciency	does not impede					node of Ranvier	CellComponent	formation of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_156_3_567_s_135	11827985	Galactolipid and MAG deficiencies impede node of Ranvier maintanence, not formation   The dramatic consequences of galactolipid and MAG elimination on nodal regions were observed around the life expectancy endpoint for this mutant line.	gene_phenotype
70092	1	333788	5	NULL	NULL	0	NULL	Ylr022cp	NucleicAcid		is required for					G1 cell cycle	Process	progression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_19_19221_s_174	15701631	Ylr022cp is required for G1 cell cycle progression.	gene_phenotype
70093	1	333790	5	NULL	NULL	0	NULL	Ylr022cp	NucleicAcid		is required for					G1 Cell Cycle	Process	progression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_19_19221_s_194	15701631	Ylr022cp Is Required for G1 Cell Cycle Progression --	gene_phenotype
70094	1	333791	5	NULL	NULL	0	NULL	YLR022C gene	GP		is essential for					cell viability	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_19_19213_s_154	15701634	Strains lacking the  YLR022C gene are not viable, indicating it is an essential gene, whereas strains lacking  YHR087W are viable ( ).	gene_phenotype
70095	2	333791	5	NULL	NULL	0	NULL	YHR087W gene	NucleicAcid		is not essential for					cell viability	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_19_19213_s_154	15701634	Strains lacking the  YLR022C gene are not viable, indicating it is an essential gene, whereas strains lacking  YHR087W are viable ( ).	gene_phenotype
70096	1	333792	5	NULL	NULL	0	NULL	YLR022C	NucleicAcid		is an orthologue of					SBDS	GP	Saccharomyces cerevisiae			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_19_19221_s_19	15701631	Haploid spores deleted for the  Saccharomyces cerevisiae SBDS orthologue  YLR022C were reported to be inviable ( ).	gene_phenotype
70097	2	333792	5	NULL	NULL	0	NULL	YLR022C	NucleicAcid		is required for					haploid spores	Cell	viability of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_19_19221_s_19	15701631	Haploid spores deleted for the  Saccharomyces cerevisiae SBDS orthologue  YLR022C were reported to be inviable ( ).	gene_phenotype
70098	1	333795	5	NULL	NULL	0	NULL	AGP2	GP		is a type of					transport protein	GP				NULL		0	NULL	NULL	NULL	gw60_embo_18_21_5843_s_9	10545096	In addition to the previously reported carnitine acetyl-CoA transferase ( CAT2), we identified the genes for the yeast orthologue of the human mitochondrial carnitine acylcarnitine translocase ( YOR100C or  CAC) and for a transport protein ( AGP2) required for carnitine transport across the plasma membrane.	gene_phenotype
70099	2	333795	5	NULL	NULL	0	NULL	carnitine	Chemical		is transported across					plasma membrane	CellComponent				NULL		0	NULL	NULL	NULL	gw60_embo_18_21_5843_s_9	10545096	In addition to the previously reported carnitine acetyl-CoA transferase ( CAT2), we identified the genes for the yeast orthologue of the human mitochondrial carnitine acylcarnitine translocase ( YOR100C or  CAC) and for a transport protein ( AGP2) required for carnitine transport across the plasma membrane.	gene_phenotype
70100	3	333795	5	NULL	NULL	0	NULL	AGP2	GP		is required for					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_21_5843_s_9	10545096	In addition to the previously reported carnitine acetyl-CoA transferase ( CAT2), we identified the genes for the yeast orthologue of the human mitochondrial carnitine acylcarnitine translocase ( YOR100C or  CAC) and for a transport protein ( AGP2) required for carnitine transport across the plasma membrane.	gene_phenotype
70101	4	333795	5	NULL	NULL	0	NULL	CAC	GP	yeast	is an orthologue of					mitochondrial carnitine acylcarnitine translocase	GP	human			NULL		0	NULL	NULL	NULL	gw60_embo_18_21_5843_s_9	10545096	In addition to the previously reported carnitine acetyl-CoA transferase ( CAT2), we identified the genes for the yeast orthologue of the human mitochondrial carnitine acylcarnitine translocase ( YOR100C or  CAC) and for a transport protein ( AGP2) required for carnitine transport across the plasma membrane.	gene_phenotype
70102	5	333795	5	NULL	NULL	0	NULL	CAT2	GP		is					carnitine acetyl-CoA transferase	GP				NULL		0	NULL	NULL	NULL	gw60_embo_18_21_5843_s_9	10545096	In addition to the previously reported carnitine acetyl-CoA transferase ( CAT2), we identified the genes for the yeast orthologue of the human mitochondrial carnitine acylcarnitine translocase ( YOR100C or  CAC) and for a transport protein ( AGP2) required for carnitine transport across the plasma membrane.	gene_phenotype
70103	6	333795	5	NULL	NULL	0	NULL	YOR100C	NucleicAcid		is the locus name of					CAC	GP				NULL		0	NULL	NULL	NULL	gw60_embo_18_21_5843_s_9	10545096	In addition to the previously reported carnitine acetyl-CoA transferase ( CAT2), we identified the genes for the yeast orthologue of the human mitochondrial carnitine acylcarnitine translocase ( YOR100C or  CAC) and for a transport protein ( AGP2) required for carnitine transport across the plasma membrane.	gene_phenotype
70104	1	333796	5	NULL	NULL	0	NULL	YOR100C gene product	GP		is a member of					mitochondrial carrier family	GP				NULL		0	NULL	NULL	NULL	gw60_embo_18_21_5843_s_111	10545096	Taken together, our experiments show that the gene product of  YOR100C is a member of the mitochondrial carrier family, which is induced on oleate, involved in the transport of acetyl-CoA from peroxisomes to mitochondria and functions as a carnitine acylcarnitine translocase in the mitochondrial inner membrane of  S.cerevisiae.	gene_phenotype
70105	2	333796	5	NULL	NULL	0	NULL	oleate	Chemical		induce					YOR100C gene product	GP				NULL		0	NULL	NULL	NULL	gw60_embo_18_21_5843_s_111	10545096	Taken together, our experiments show that the gene product of  YOR100C is a member of the mitochondrial carrier family, which is induced on oleate, involved in the transport of acetyl-CoA from peroxisomes to mitochondria and functions as a carnitine acylcarnitine translocase in the mitochondrial inner membrane of  S.cerevisiae.	gene_phenotype
70106	3	333796	5	NULL	NULL	0	NULL	acetyl-CoA	GP		is transported from					peroxisomes	CellComponent				NULL		0	NULL	NULL	NULL	gw60_embo_18_21_5843_s_111	10545096	Taken together, our experiments show that the gene product of  YOR100C is a member of the mitochondrial carrier family, which is induced on oleate, involved in the transport of acetyl-CoA from peroxisomes to mitochondria and functions as a carnitine acylcarnitine translocase in the mitochondrial inner membrane of  S.cerevisiae.	gene_phenotype
70107	4	333796	5	NULL	NULL	0	NULL	acetyl-CoA	GP		is transported to					mitochondria	CellComponent				NULL		0	NULL	NULL	NULL	gw60_embo_18_21_5843_s_111	10545096	Taken together, our experiments show that the gene product of  YOR100C is a member of the mitochondrial carrier family, which is induced on oleate, involved in the transport of acetyl-CoA from peroxisomes to mitochondria and functions as a carnitine acylcarnitine translocase in the mitochondrial inner membrane of  S.cerevisiae.	gene_phenotype
70108	5	333796	5	NULL	NULL	0	NULL	statement 3	Process		occurs along with					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_21_5843_s_111	10545096	Taken together, our experiments show that the gene product of  YOR100C is a member of the mitochondrial carrier family, which is induced on oleate, involved in the transport of acetyl-CoA from peroxisomes to mitochondria and functions as a carnitine acylcarnitine translocase in the mitochondrial inner membrane of  S.cerevisiae.	gene_phenotype
70109	6	333796	5	NULL	NULL	0	NULL	YOR100C gene product	GP		is involved in					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_21_5843_s_111	10545096	Taken together, our experiments show that the gene product of  YOR100C is a member of the mitochondrial carrier family, which is induced on oleate, involved in the transport of acetyl-CoA from peroxisomes to mitochondria and functions as a carnitine acylcarnitine translocase in the mitochondrial inner membrane of  S.cerevisiae.	gene_phenotype
70110	7	333796	5	NULL	NULL	0	NULL	YOR100C gene product	GP		is involved in					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_21_5843_s_111	10545096	Taken together, our experiments show that the gene product of  YOR100C is a member of the mitochondrial carrier family, which is induced on oleate, involved in the transport of acetyl-CoA from peroxisomes to mitochondria and functions as a carnitine acylcarnitine translocase in the mitochondrial inner membrane of  S.cerevisiae.	gene_phenotype
70111	8	333796	5	NULL	NULL	0	NULL	YOR100C gene product	GP		functions as					carnitine acylcarnitine translocase	GP				NULL	mitochondrial inner membrane of S.cerevisiae.	0	NULL	NULL	NULL	gw60_embo_18_21_5843_s_111	10545096	Taken together, our experiments show that the gene product of  YOR100C is a member of the mitochondrial carrier family, which is induced on oleate, involved in the transport of acetyl-CoA from peroxisomes to mitochondria and functions as a carnitine acylcarnitine translocase in the mitochondrial inner membrane of  S.cerevisiae.	gene_phenotype
70121	1	333797	5	NULL	NULL	0	NULL	ORF YBL064C protein	GP		is homologous to					peroxiredoxins	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_16296_s_216	10821871	The protein coded by the ORF YBL064C showed homology to peroxiredoxins and had a potential mitochondrial targeting signal, and although the product of ORF YBL064C belongs to the 1-Cys Prx group, we decided to test whether it had specific TPx activity with the mitochondrial thioredoxin system.	gene_phenotype
70122	2	333797	5	NULL	NULL	0	NULL	ORF YBL064C protein	GP		contains					mitochondrial targeting signal	AminoAcid	potential			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_16296_s_216	10821871	The protein coded by the ORF YBL064C showed homology to peroxiredoxins and had a potential mitochondrial targeting signal, and although the product of ORF YBL064C belongs to the 1-Cys Prx group, we decided to test whether it had specific TPx activity with the mitochondrial thioredoxin system.	gene_phenotype
70123	3	333797	5	NULL	NULL	0	NULL	ORF YBL064C protein	GP		belongs tp					1-Cys Prx group	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_16296_s_216	10821871	The protein coded by the ORF YBL064C showed homology to peroxiredoxins and had a potential mitochondrial targeting signal, and although the product of ORF YBL064C belongs to the 1-Cys Prx group, we decided to test whether it had specific TPx activity with the mitochondrial thioredoxin system.	gene_phenotype
70125	4	333797	5	NULL	NULL	NULL	NULL	ORF YBL064C protein	GP		activates		potentially			TPx	GP				NULL	mitochondrial thioredoxin system	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_16296_s_216	10821871	The protein coded by the ORF YBL064C showed homology to peroxiredoxins and had a potential mitochondrial targeting signal, and although the product of ORF YBL064C belongs to the 1-Cys Prx group, we decided to test whether it had specific TPx activity with the mitochondrial thioredoxin system.	gene_phenotype
70126	1	333799	5	NULL	NULL	0	NULL	YGR024c	NucleicAcid		is a type of					ORF	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_genesdev_17_23_2889_s_118	14633974	THG1 (ORF YGR024c) encodes a protein with tRNAHis guanylyltransferase activity	gene_phenotype
70127	2	333799	5	NULL	NULL	0	NULL	YGR024c	NucleicAcid		is the locus name of					THG1	GP				NULL		0	NULL	NULL	NULL	gw70_genesdev_17_23_2889_s_118	14633974	THG1 (ORF YGR024c) encodes a protein with tRNAHis guanylyltransferase activity	gene_phenotype
70128	3	333799	5	NULL	NULL	0	NULL	THG1	GP		activates					tRNAHis guanylyltransferase	GP				NULL		0	NULL	NULL	NULL	gw70_genesdev_17_23_2889_s_118	14633974	THG1 (ORF YGR024c) encodes a protein with tRNAHis guanylyltransferase activity	gene_phenotype
70129	1	333800	5	NULL	NULL	0	NULL	YGR024c	NucleicAcid		is a type of					ORF	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_genesdev_17_23_2889_s_41	14633974	Using a previously described biochemical genomics approach (Martzen et al. 1999 ), and an assay based on incorporation of [alpha-32]GTP into a tRNAHis substrate, we identified a 28-kD protein, encoded by the essential ORF YGR024c, that copurifies with tRNAHis guanylyltransferase activity.	gene_phenotype
70130	2	333800	5	NULL	NULL	0	NULL	YGR024c protein	GP		activates					tRNAHis guanylyltransferase	GP				NULL		0	NULL	NULL	NULL	gw70_genesdev_17_23_2889_s_41	14633974	Using a previously described biochemical genomics approach (Martzen et al. 1999 ), and an assay based on incorporation of [alpha-32]GTP into a tRNAHis substrate, we identified a 28-kD protein, encoded by the essential ORF YGR024c, that copurifies with tRNAHis guanylyltransferase activity.	gene_phenotype
70131	1	333801	5	NULL	NULL	0	NULL	YJR019C	NucleicAcid		is renamed as					PTE1	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_14_9216_s_247	10092594	We propose that  YJR019C and human  hTE both be renamed  PTE1 to reflect the peroxisomal distribution and acyl-CoA thioesterase activity of their gene products.	gene_phenotype
70132	2	333801	5	NULL	NULL	0	NULL	hTE	GP	human	is renamed as					PTE1	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_14_9216_s_247	10092594	We propose that  YJR019C and human  hTE both be renamed  PTE1 to reflect the peroxisomal distribution and acyl-CoA thioesterase activity of their gene products.	gene_phenotype
70133	3	333801	5	NULL	NULL	0	NULL	PTE1	GP		distributed in					peroxisome	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_14_9216_s_247	10092594	We propose that  YJR019C and human  hTE both be renamed  PTE1 to reflect the peroxisomal distribution and acyl-CoA thioesterase activity of their gene products.	gene_phenotype
70134	4	333801	5	NULL	NULL	0	NULL	PTE1	GP		activates					acyl-CoA thioesterase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_14_9216_s_247	10092594	We propose that  YJR019C and human  hTE both be renamed  PTE1 to reflect the peroxisomal distribution and acyl-CoA thioesterase activity of their gene products.	gene_phenotype
70135	1	333803	5	NULL	NULL	0	NULL	YKL187c	NucleicAcid		is linked to		probably			succinate dehydrogenase	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_23_7_553_s_386	16710832	YKL187c is linked to a probable succinate dehydrogenase by STRING and annotated to  15 terms ( p > 0.25) by GeneFAS (cell growth and/or maintenance, metabolism, organic acid metabolism,  energy pathways, transport, electron transport, phosphorus metabolism, cell communication,  carboxylic acid metabolism, carbohydrate metabolism, energy derivation by oxidation  of organic compounds, coenzymes and prosthetic group metabolism, signal transduction,  oxidative phosphorylation, phosphate metabolism, response to stress, main pathways  of carbohydrate metabolism, phosphorylation biosynthesis, TCA intermediate metabolism,  main pathways of carbohydrate metabolism, amine metabolism, amino acid and derivative  metabolism, tricarboxylic acid cycle, and lipid metabolism), most of which are related  to the un-supported  carbohydrate and alcohol metabolism  annotation made in this study.	gene_phenotype
70146	1	333805	5	NULL	NULL	0	NULL	YLR011wp protein	GP		activates					reductase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34890_s_238	15184374	The biochemical studies aimed to identify YLR011wp  in vivo activity showed that the protein bears several reductase activities that are NAD(P)H-dependent and involve FMN as a cofactor.	gene_phenotype
70147	2	333805	5	NULL	NULL	0	NULL	statement 1	Process		is dependent on					NAD(P)H	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34890_s_238	15184374	The biochemical studies aimed to identify YLR011wp  in vivo activity showed that the protein bears several reductase activities that are NAD(P)H-dependent and involve FMN as a cofactor.	gene_phenotype
70148	3	333805	5	NULL	NULL	0	NULL	statement 1	Process		involves					FMN	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34890_s_238	15184374	The biochemical studies aimed to identify YLR011wp  in vivo activity showed that the protein bears several reductase activities that are NAD(P)H-dependent and involve FMN as a cofactor.	gene_phenotype
70149	4	333805	5	NULL	NULL	0	NULL	FMN	Chemical		acts as					cofactor	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34890_s_238	15184374	The biochemical studies aimed to identify YLR011wp  in vivo activity showed that the protein bears several reductase activities that are NAD(P)H-dependent and involve FMN as a cofactor.	gene_phenotype
70150	1	333806	5	NULL	NULL	NULL	NULL	YLR011wp	NucleicAcid		is an acceptor of		natural			electron transfer	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_33_34890_s_183	15184374	Therefore, if YLR011wp has a natural acceptor for electron transfer via FMN, the FMN reductase activity detected reflects either the reduction of free oxidized FMN via enzyme-bound FMN ( Fig. 5 b) or the rapid exchange reaction between the reduced and oxidized forms of FMN at the protein FMN binding site ( Fig. 5 c).	gene_phenotype
70151	2	333806	5	NULL	NULL	0	NULL	statement 1	Process		via					FMN	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34890_s_183	15184374	Therefore, if YLR011wp has a natural acceptor for electron transfer via FMN, the FMN reductase activity detected reflects either the reduction of free oxidized FMN via enzyme-bound FMN ( Fig. 5 b) or the rapid exchange reaction between the reduced and oxidized forms of FMN at the protein FMN binding site ( Fig. 5 c).	gene_phenotype
70153	3	333806	5	NULL	NULL	0	NULL	YLR011wp	NucleicAcid		activates					FMN reductase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34890_s_183	15184374	Therefore, if YLR011wp has a natural acceptor for electron transfer via FMN, the FMN reductase activity detected reflects either the reduction of free oxidized FMN via enzyme-bound FMN ( Fig. 5 b) or the rapid exchange reaction between the reduced and oxidized forms of FMN at the protein FMN binding site ( Fig. 5 c).	gene_phenotype
70156	4	333806	5	NULL	NULL	NULL	NULL	FMN	Chemical	free;;oxidized	undergoes					reduction	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_33_34890_s_183	15184374	Therefore, if YLR011wp has a natural acceptor for electron transfer via FMN, the FMN reductase activity detected reflects either the reduction of free oxidized FMN via enzyme-bound FMN ( Fig. 5 b) or the rapid exchange reaction between the reduced and oxidized forms of FMN at the protein FMN binding site ( Fig. 5 c).	gene_phenotype
70157	5	333806	5	NULL	NULL	0	NULL	statement 4	Process		via					enzyme-bound FMN	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34890_s_183	15184374	Therefore, if YLR011wp has a natural acceptor for electron transfer via FMN, the FMN reductase activity detected reflects either the reduction of free oxidized FMN via enzyme-bound FMN ( Fig. 5 b) or the rapid exchange reaction between the reduced and oxidized forms of FMN at the protein FMN binding site ( Fig. 5 c).	gene_phenotype
70158	6	333806	5	NULL	NULL	0	NULL	FMN	Chemical	reduced	is exchanged with					FMN	Chemical	oxidized			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34890_s_183	15184374	Therefore, if YLR011wp has a natural acceptor for electron transfer via FMN, the FMN reductase activity detected reflects either the reduction of free oxidized FMN via enzyme-bound FMN ( Fig. 5 b) or the rapid exchange reaction between the reduced and oxidized forms of FMN at the protein FMN binding site ( Fig. 5 c).	gene_phenotype
70159	7	333806	5	NULL	NULL	0	NULL	statement 6	Process		occurs at					protein FMN binding site	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34890_s_183	15184374	Therefore, if YLR011wp has a natural acceptor for electron transfer via FMN, the FMN reductase activity detected reflects either the reduction of free oxidized FMN via enzyme-bound FMN ( Fig. 5 b) or the rapid exchange reaction between the reduced and oxidized forms of FMN at the protein FMN binding site ( Fig. 5 c).	gene_phenotype
70160	8	333806	5	NULL	NULL	0	NULL	statement 6	Process		is a type of					rapid exchange reaction	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34890_s_183	15184374	Therefore, if YLR011wp has a natural acceptor for electron transfer via FMN, the FMN reductase activity detected reflects either the reduction of free oxidized FMN via enzyme-bound FMN ( Fig. 5 b) or the rapid exchange reaction between the reduced and oxidized forms of FMN at the protein FMN binding site ( Fig. 5 c).	gene_phenotype
70161	9	333806	5	NULL	NULL	0	NULL	statement 3	Process		reflects					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34890_s_183	15184374	Therefore, if YLR011wp has a natural acceptor for electron transfer via FMN, the FMN reductase activity detected reflects either the reduction of free oxidized FMN via enzyme-bound FMN ( Fig. 5 b) or the rapid exchange reaction between the reduced and oxidized forms of FMN at the protein FMN binding site ( Fig. 5 c).	gene_phenotype
70162	10	333806	5	NULL	NULL	0	NULL	statement 3	Process		reflects					statement 6	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34890_s_183	15184374	Therefore, if YLR011wp has a natural acceptor for electron transfer via FMN, the FMN reductase activity detected reflects either the reduction of free oxidized FMN via enzyme-bound FMN ( Fig. 5 b) or the rapid exchange reaction between the reduced and oxidized forms of FMN at the protein FMN binding site ( Fig. 5 c).	gene_phenotype
70163	11	333806	5	NULL	NULL	0	NULL	statement 9	Process		is an alternative to					statement 10	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34890_s_183	15184374	Therefore, if YLR011wp has a natural acceptor for electron transfer via FMN, the FMN reductase activity detected reflects either the reduction of free oxidized FMN via enzyme-bound FMN ( Fig. 5 b) or the rapid exchange reaction between the reduced and oxidized forms of FMN at the protein FMN binding site ( Fig. 5 c).	gene_phenotype
70164	1	333811	5	NULL	NULL	0	NULL	Ypr128cp	NucleicAcid		is the locus name of					Ant1p	GP				NULL		0	NULL	NULL	NULL	gw60_embo_20_18_5049_s_3	11566870	Here we report the identification and functional reconstitution of Ant1p (Ypr128cp), a peroxisomal transporter in the yeast  Saccharomyces cerevisiae, which has the characteristic sequence features of the mitochondrial carrier family.	gene_phenotype
70165	2	333811	5	NULL	NULL	0	NULL	Ant1p	GP		is a type of					peroxisomal transporter	GP				NULL	yeast Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw60_embo_20_18_5049_s_3	11566870	Here we report the identification and functional reconstitution of Ant1p (Ypr128cp), a peroxisomal transporter in the yeast  Saccharomyces cerevisiae, which has the characteristic sequence features of the mitochondrial carrier family.	gene_phenotype
70166	3	333811	5	NULL	NULL	0	NULL	Ant1p 	GP	sequence features of	is characteristic to					mitochondrial carrier family	GP				NULL		0	NULL	NULL	NULL	gw60_embo_20_18_5049_s_3	11566870	Here we report the identification and functional reconstitution of Ant1p (Ypr128cp), a peroxisomal transporter in the yeast  Saccharomyces cerevisiae, which has the characteristic sequence features of the mitochondrial carrier family.	gene_phenotype
70167	2	333815	5	NULL	NULL	NULL	NULL	QAOS	MedicalProcedure		measures					statement 1	Process				NULL	in vivo in budding yeast cdc13 mutants	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_21_4414_s_119	11691929	The data in the right lanes of Figure  1B are in complete agreement with our previous findings and show that QAOS is capable of measuring ssDNA produced at  YER186C in vivo, in budding yeast  cdc13 mutants.	gene_phenotype
70168	1	333815	5	NULL	NULL	NULL	NULL	ssDNA	NucleicAcid		is produced at					YER186C	NucleicAcid				NULL	in vivo in budding yeast cdc13 mutants	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_21_4414_s_119	11691929	The data in the right lanes of Figure  1B are in complete agreement with our previous findings and show that QAOS is capable of measuring ssDNA produced at  YER186C in vivo, in budding yeast  cdc13 mutants.	gene_phenotype
70169	1	333817	5	NULL	NULL	0	NULL	YAL061W	NucleicAcid		is a type of					sporulation gene	GP				NULL		0	NULL	NULL	NULL	gw60_genetics_163_1_47_s_114	12586695	YAL061W is a representative essential sporulation gene and the deletion mutant shows an  IME1 expression phenotype consistent with an arrest after  IME1 induction.	gene_phenotype
70170	2	333817	5	NULL	NULL	0	NULL	YAL061W	NucleicAcid	deletion mutant	shows					IME1 expression phenotype	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	gw60_genetics_163_1_47_s_114	12586695	YAL061W is a representative essential sporulation gene and the deletion mutant shows an  IME1 expression phenotype consistent with an arrest after  IME1 induction.	gene_phenotype
70171	3	333817	5	NULL	NULL	0	NULL	arrest	Process		occurs after					IME1	GP	induction of			NULL		0	NULL	NULL	NULL	gw60_genetics_163_1_47_s_114	12586695	YAL061W is a representative essential sporulation gene and the deletion mutant shows an  IME1 expression phenotype consistent with an arrest after  IME1 induction.	gene_phenotype
70172	4	333817	5	NULL	NULL	0	NULL	statement 2	Process		consistent with					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_163_1_47_s_114	12586695	YAL061W is a representative essential sporulation gene and the deletion mutant shows an  IME1 expression phenotype consistent with an arrest after  IME1 induction.	gene_phenotype
70173	1	333818	5	NULL	NULL	0	NULL	YHR087W orthologue	GP	S. pombe	is expressed during					sporulation	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_19_19213_s_112	15701634	This protein did not have a previously known structure or function; however, the YHR087W orthologue in  S. pombe is expressed during sporulation and environmental stress ( ,  ).	gene_phenotype
70174	2	333818	5	NULL	NULL	0	NULL	YHR087W orthologue	GP	S. pombe	is expressed during					environmental stress	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_19_19213_s_112	15701634	This protein did not have a previously known structure or function; however, the YHR087W orthologue in  S. pombe is expressed during sporulation and environmental stress ( ,  ).	gene_phenotype
70175	1	333819	5	NULL	NULL	0	NULL	YER158c	NucleicAcid		regulates		possibly			pheromone signaling	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_155_1_43_s_256	10790383	To determine whether  YER158c can regulate pheromone signaling, cells carrying the  YER158c sequences cloned into a 2mu multicopy vector were assayed for their sensitivity to alpha-factor in a halo assay ( Fig 8).	gene_phenotype
70176	1	333820	5	NULL	NULL	0	NULL	Kss1	GP		is a type of					MAP kinase	GP				NULL		0	NULL	NULL	NULL	gw70_genomeres_15_4_560_s_90	15805496	Sequencing revealed six proteins: Kss1, the MAP kinase for the filamentous growth pathway; Tpk2, a cAMP-dependent kinase subunit; Gis2, an uncharacterized protein involved in glucose sensing; Ypc1, a ceramidase enzyme; and two uncharacterized proteins, Yer158c and Ybr062c.	gene_phenotype
70177	2	333820	5	NULL	NULL	0	NULL	Kss1	GP		is involved in					filamentous growth pathway	Process				NULL		0	NULL	NULL	NULL	gw70_genomeres_15_4_560_s_90	15805496	Sequencing revealed six proteins: Kss1, the MAP kinase for the filamentous growth pathway; Tpk2, a cAMP-dependent kinase subunit; Gis2, an uncharacterized protein involved in glucose sensing; Ypc1, a ceramidase enzyme; and two uncharacterized proteins, Yer158c and Ybr062c.	gene_phenotype
70178	3	333820	5	NULL	NULL	0	NULL	Tpk2	GP		is a type of					cAMP-dependent kinase subunit	GP				NULL		0	NULL	NULL	NULL	gw70_genomeres_15_4_560_s_90	15805496	Sequencing revealed six proteins: Kss1, the MAP kinase for the filamentous growth pathway; Tpk2, a cAMP-dependent kinase subunit; Gis2, an uncharacterized protein involved in glucose sensing; Ypc1, a ceramidase enzyme; and two uncharacterized proteins, Yer158c and Ybr062c.	gene_phenotype
70179	4	333820	5	NULL	NULL	0	NULL	Gis2	GP		is involved in					glucose	Chemical	sensing of			NULL		0	NULL	NULL	NULL	gw70_genomeres_15_4_560_s_90	15805496	Sequencing revealed six proteins: Kss1, the MAP kinase for the filamentous growth pathway; Tpk2, a cAMP-dependent kinase subunit; Gis2, an uncharacterized protein involved in glucose sensing; Ypc1, a ceramidase enzyme; and two uncharacterized proteins, Yer158c and Ybr062c.	gene_phenotype
70180	5	333820	5	NULL	NULL	0	NULL	Ypc1	GP		is a type of					ceramidase enzyme	GP				NULL		0	NULL	NULL	NULL	gw70_genomeres_15_4_560_s_90	15805496	Sequencing revealed six proteins: Kss1, the MAP kinase for the filamentous growth pathway; Tpk2, a cAMP-dependent kinase subunit; Gis2, an uncharacterized protein involved in glucose sensing; Ypc1, a ceramidase enzyme; and two uncharacterized proteins, Yer158c and Ybr062c.	gene_phenotype
70181	1	333821	5	NULL	NULL	0	NULL	YER158c	NucleicAcid	expression of	is not regulated by					cell cycle	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_155_1_43_s_252	10790383	DNA microarray analysis indicates that  YER158c expression is not cell cycle regulated ( S MITH et al. 1996   ;   S PELLMAN et al. 1998   ), is induced during diauxic growth ( D ERISI et al. 1997   ), and is repressed during sporulation ( C HU et al. 1998   ).	gene_phenotype
70182	2	333821	5	NULL	NULL	0	NULL	YER158c	NucleicAcid	expression of	is induced during					diauxic growth	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_155_1_43_s_252	10790383	DNA microarray analysis indicates that  YER158c expression is not cell cycle regulated ( S MITH et al. 1996   ;   S PELLMAN et al. 1998   ), is induced during diauxic growth ( D ERISI et al. 1997   ), and is repressed during sporulation ( C HU et al. 1998   ).	gene_phenotype
70183	3	333821	5	NULL	NULL	0	NULL	YER158c	NucleicAcid	expression of	is repressed during					sporulation	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_155_1_43_s_252	10790383	DNA microarray analysis indicates that  YER158c expression is not cell cycle regulated ( S MITH et al. 1996   ;   S PELLMAN et al. 1998   ), is induced during diauxic growth ( D ERISI et al. 1997   ), and is repressed during sporulation ( C HU et al. 1998   ).	gene_phenotype
70184	2	333824	5	NULL	NULL	NULL	NULL	peroxisomes	CellComponent	yeast	activates					delta3,delta2-enoyl-CoA isomerase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33184_s_225	9837886	Although a prior report suggested that the delta3,delta2-enoyl-CoA isomerase activity of yeast peroxisomes is an intrinsic feature of acyl-CoA oxidase (Pox1) ( 35), our findings demonstrate that this activity is dependent on the protein encoded by  YLR284C.	gene_phenotype
70185	1	333824	5	NULL	NULL	NULL	NULL	acyl-CoA oxidase	GP		is a synonym of					Pox1	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_50_33184_s_225	9837886	Although a prior report suggested that the delta3,delta2-enoyl-CoA isomerase activity of yeast peroxisomes is an intrinsic feature of acyl-CoA oxidase (Pox1) ( 35), our findings demonstrate that this activity is dependent on the protein encoded by  YLR284C.	gene_phenotype
70186	3	333824	5	NULL	NULL	0	NULL	statement 2	Process		is an intrinsic feature of					acyl-CoA oxidase 	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_50_33184_s_225	9837886	Although a prior report suggested that the delta3,delta2-enoyl-CoA isomerase activity of yeast peroxisomes is an intrinsic feature of acyl-CoA oxidase (Pox1) ( 35), our findings demonstrate that this activity is dependent on the protein encoded by  YLR284C.	gene_phenotype
70187	4	333824	5	NULL	NULL	0	NULL	statement 2	Process		is dependent on					YLR284C protein	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_50_33184_s_225	9837886	Although a prior report suggested that the delta3,delta2-enoyl-CoA isomerase activity of yeast peroxisomes is an intrinsic feature of acyl-CoA oxidase (Pox1) ( 35), our findings demonstrate that this activity is dependent on the protein encoded by  YLR284C.	gene_phenotype
70188	1	333825	5	NULL	NULL	0	NULL	YOL151w	NucleicAcid		is the locus name of					GRE2	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_20_6_545_s_231	12722185	We conclude that GRE2/YOL151w, but not YDR541c, YGL039w or YGL157w, encodes a  protein with methylglyoxal-reducing activity.	gene_phenotype
70189	2	333825	5	NULL	NULL	0	NULL	GRE2	GP		activates					methylglyoxal	Chemical	reduction of			NULL		0	NULL	NULL	NULL	gw70_yeast_20_6_545_s_231	12722185	We conclude that GRE2/YOL151w, but not YDR541c, YGL039w or YGL157w, encodes a  protein with methylglyoxal-reducing activity.	gene_phenotype
70190	3	333825	5	NULL	NULL	0	NULL	YDR541c protein	GP		does not activate					methylglyoxal	Chemical	reduction of			NULL		0	NULL	NULL	NULL	gw70_yeast_20_6_545_s_231	12722185	We conclude that GRE2/YOL151w, but not YDR541c, YGL039w or YGL157w, encodes a  protein with methylglyoxal-reducing activity.	gene_phenotype
70191	4	333825	5	NULL	NULL	0	NULL	YGL039w protein	GP		does not activate					methylglyoxal	Chemical	reduction of			NULL		0	NULL	NULL	NULL	gw70_yeast_20_6_545_s_231	12722185	We conclude that GRE2/YOL151w, but not YDR541c, YGL039w or YGL157w, encodes a  protein with methylglyoxal-reducing activity.	gene_phenotype
70192	5	333825	5	NULL	NULL	0	NULL	YGL157w protein	GP		activates					methylglyoxal	Chemical	reduction of			NULL		0	NULL	NULL	NULL	gw70_yeast_20_6_545_s_231	12722185	We conclude that GRE2/YOL151w, but not YDR541c, YGL039w or YGL157w, encodes a  protein with methylglyoxal-reducing activity.	gene_phenotype
70193	1	333827	5	NULL	NULL	0	NULL	YHR150w	NucleicAcid		encodes					peroxisomal integral membrane proteins	GP				NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw70_cellbiol_161_2_321_s_1	12707309	YHR150w and YDR479c encode peroxisomal integral membrane proteins involved in the regulation of peroxisome number, size, and distribution in Saccharomyces cerevisiae.	gene_phenotype
70194	2	333827	5	NULL	NULL	0	NULL	YDR479c	NucleicAcid		encodes					peroxisomal integral membrane proteins	GP				NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw70_cellbiol_161_2_321_s_1	12707309	YHR150w and YDR479c encode peroxisomal integral membrane proteins involved in the regulation of peroxisome number, size, and distribution in Saccharomyces cerevisiae.	gene_phenotype
70195	3	333827	5	NULL	NULL	0	NULL	peroxisomal integral membrane proteins	GP		regulates					peroxisome	CellComponent	number of			NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw70_cellbiol_161_2_321_s_1	12707309	YHR150w and YDR479c encode peroxisomal integral membrane proteins involved in the regulation of peroxisome number, size, and distribution in Saccharomyces cerevisiae.	gene_phenotype
70196	4	333827	5	NULL	NULL	0	NULL	peroxisomal integral membrane proteins	GP		regulates					peroxisome	CellComponent	size of			NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw70_cellbiol_161_2_321_s_1	12707309	YHR150w and YDR479c encode peroxisomal integral membrane proteins involved in the regulation of peroxisome number, size, and distribution in Saccharomyces cerevisiae.	gene_phenotype
70197	5	333827	5	NULL	NULL	0	NULL	peroxisomal integral membrane proteins	GP		regulates					peroxisome	CellComponent	distribution of			NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw70_cellbiol_161_2_321_s_1	12707309	YHR150w and YDR479c encode peroxisomal integral membrane proteins involved in the regulation of peroxisome number, size, and distribution in Saccharomyces cerevisiae.	gene_phenotype
70198	1	333828	5	NULL	NULL	0	NULL	YHR150w	NucleicAcid		controls					peroxisome	CellComponent	size of			NULL		0	NULL	NULL	NULL	gw70_cellbiol_161_2_321_s_183	12707309	These characteristics of peroxisomes of the deletion strains are consistent with a role for  YHR150w and  YDR479c in the control of peroxisome size, number, and distribution within cells.	gene_phenotype
70199	2	333828	5	NULL	NULL	0	NULL	YHR150w	NucleicAcid		controls					peroxisome	CellComponent	number of			NULL		0	NULL	NULL	NULL	gw70_cellbiol_161_2_321_s_183	12707309	These characteristics of peroxisomes of the deletion strains are consistent with a role for  YHR150w and  YDR479c in the control of peroxisome size, number, and distribution within cells.	gene_phenotype
70200	3	333828	5	NULL	NULL	0	NULL	YHR150w	NucleicAcid		controls					peroxisome	CellComponent	distribution of			NULL		0	NULL	NULL	NULL	gw70_cellbiol_161_2_321_s_183	12707309	These characteristics of peroxisomes of the deletion strains are consistent with a role for  YHR150w and  YDR479c in the control of peroxisome size, number, and distribution within cells.	gene_phenotype
70201	4	333828	5	NULL	NULL	0	NULL	YDR479c	NucleicAcid		controls					peroxisome	CellComponent	size of			NULL		0	NULL	NULL	NULL	gw70_cellbiol_161_2_321_s_183	12707309	These characteristics of peroxisomes of the deletion strains are consistent with a role for  YHR150w and  YDR479c in the control of peroxisome size, number, and distribution within cells.	gene_phenotype
70202	5	333828	5	NULL	NULL	0	NULL	YDR479c	NucleicAcid		controls					peroxisome	CellComponent	number of			NULL		0	NULL	NULL	NULL	gw70_cellbiol_161_2_321_s_183	12707309	These characteristics of peroxisomes of the deletion strains are consistent with a role for  YHR150w and  YDR479c in the control of peroxisome size, number, and distribution within cells.	gene_phenotype
70203	6	333828	5	NULL	NULL	0	NULL	YDR479c	NucleicAcid		controls					peroxisome	CellComponent	distribution of			NULL		0	NULL	NULL	NULL	gw70_cellbiol_161_2_321_s_183	12707309	These characteristics of peroxisomes of the deletion strains are consistent with a role for  YHR150w and  YDR479c in the control of peroxisome size, number, and distribution within cells.	gene_phenotype
70213	1	333834	5	NULL	NULL	0	NULL	YNL063w protein	GP		does not activate					protoporphyrinogen	GP				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_173_1_175_s_150	10220893	Biochemical analysis and complementation assays provide evidence that the protein encoded by YNL063w is not involved in protoporphyrinogen activity.	gene_phenotype
70214	1	333835	5	NULL	NULL	0	NULL	YNL063w protein	GP	S. cerevisiae	does not activate					protoporphyrinogen	GP				NULL		0	NULL	NULL	NULL	gw60_embo_21_4_769_s_183	11847124	A functional analysis of the  S. cerevisiaeprotein, called YNL063w, concluded that it did not possess protoporphyrinogen activity ( Le Guen  et al., 1999), thought to be the role of the  E.coli HemK protein ( Nakayashiki  et al., 1995).	gene_phenotype
70215	2	333835	5	NULL	NULL	0	NULL	YNL063w protein	GP	S. cerevisiae	plays a role as		possibly			HemK protein	GP	E.coli			NULL		0	NULL	NULL	NULL	gw60_embo_21_4_769_s_183	11847124	A functional analysis of the  S. cerevisiaeprotein, called YNL063w, concluded that it did not possess protoporphyrinogen activity ( Le Guen  et al., 1999), thought to be the role of the  E.coli HemK protein ( Nakayashiki  et al., 1995).	gene_phenotype
70216	1	333836	5	NULL	NULL	0	NULL	ORF YNL063w product	GP		is similar to					hemK gene	GP	E.coli			NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_173_1_175_s_25	10220893	In order to find out whether the product of the ORF YNL063w, which is similar to the  hemK gene of  E. coli, is also involved in the protoporphyrinogen oxidase activity, we investigated the possible role in heme synthesis of this protein in yeast.	gene_phenotype
70218	2	333836	5	NULL	NULL	0	NULL	ORF YNL063w product	GP		activates		potentially			protoporphyrinogen oxidase	GP				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_173_1_175_s_25	10220893	In order to find out whether the product of the ORF YNL063w, which is similar to the  hemK gene of  E. coli, is also involved in the protoporphyrinogen oxidase activity, we investigated the possible role in heme synthesis of this protein in yeast.	gene_phenotype
70219	1	333837	5	NULL	NULL	0	NULL	YLR127c	NucleicAcid		encodes		possibly			APC subunit	GP	budding yeast			NULL		0	NULL	NULL	NULL	gw60_science_279_5354_1219_s_61	9469815	To determine whether YLR127c encodes an APC subunit in budding yeast, we cloned the gene encoding YLR127c and inserted a triple hemagglutinin (HA) epitope tag at the NH2-terminus ( 26).	gene_phenotype
70230	1	333839	5	NULL	NULL	0	NULL	IPTG	Chemical	application of	leads to					ATP/ADP transporter		presence of;;functional			NULL	cytoplasmic membrane of E. coli harboring plasmid pET6 	0	NULL	NULL	NULL	gw60_jbiolchem_273_16_9630_s_187	9545295	As the data above clearly show that IPTG application to  E. coli harboring plasmid pET6 leads to the presence of a functional ATP/ADP transporter in the cytoplasmic bacterial membrane it was tempting to analyze IPTG-induced protein synthesis in more detail.	gene_phenotype
70311	1	333840	5	NULL	NULL	0	NULL	Yor145c protein	GP		is a type of					nucleolar protein	GP				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_31_10_2524_s_2	12736301	A strain of  Saccharomyces cerevisiae, defective in small subunit ribosomal RNA processing, has a mutation in  YOR145c ORF that converts Gly235 to Asp. Yor145c is a nucleolar protein required for cell viability and has been reported recently to be present in 90S pre-ribosomal particles.	gene_phenotype
70312	2	333840	5	NULL	NULL	0	NULL	Yor145c protein	GP		is required for					cell viability	Process				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_31_10_2524_s_2	12736301	A strain of  Saccharomyces cerevisiae, defective in small subunit ribosomal RNA processing, has a mutation in  YOR145c ORF that converts Gly235 to Asp. Yor145c is a nucleolar protein required for cell viability and has been reported recently to be present in 90S pre-ribosomal particles.	gene_phenotype
70313	3	333840	5	NULL	NULL	0	NULL	Yor145c protein	GP		is present in					90S pre-ribosomal particles	GP				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_31_10_2524_s_2	12736301	A strain of  Saccharomyces cerevisiae, defective in small subunit ribosomal RNA processing, has a mutation in  YOR145c ORF that converts Gly235 to Asp. Yor145c is a nucleolar protein required for cell viability and has been reported recently to be present in 90S pre-ribosomal particles.	gene_phenotype
70314	4	333840	5	NULL	NULL	0	NULL	Gly235	AminoAcid		is converted to					Asp	AminoAcid				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_31_10_2524_s_2	12736301	A strain of  Saccharomyces cerevisiae, defective in small subunit ribosomal RNA processing, has a mutation in  YOR145c ORF that converts Gly235 to Asp. Yor145c is a nucleolar protein required for cell viability and has been reported recently to be present in 90S pre-ribosomal particles.	gene_phenotype
70315	5	333840	5	NULL	NULL	0	NULL	YOR145c ORF	NucleicAcid	mutant	is required for					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_31_10_2524_s_2	12736301	A strain of  Saccharomyces cerevisiae, defective in small subunit ribosomal RNA processing, has a mutation in  YOR145c ORF that converts Gly235 to Asp. Yor145c is a nucleolar protein required for cell viability and has been reported recently to be present in 90S pre-ribosomal particles.	gene_phenotype
70316	6	333840	5	NULL	NULL	0	NULL	Saccharomyces cerevisiae strain	Organism		is defective in					small subunit ribosomal RNA	NucleicAcid	processing of			NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_31_10_2524_s_2	12736301	A strain of  Saccharomyces cerevisiae, defective in small subunit ribosomal RNA processing, has a mutation in  YOR145c ORF that converts Gly235 to Asp. Yor145c is a nucleolar protein required for cell viability and has been reported recently to be present in 90S pre-ribosomal particles.	gene_phenotype
70317	7	333840	5	NULL	NULL	0	NULL	statement 6	Process		contains					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_31_10_2524_s_2	12736301	A strain of  Saccharomyces cerevisiae, defective in small subunit ribosomal RNA processing, has a mutation in  YOR145c ORF that converts Gly235 to Asp. Yor145c is a nucleolar protein required for cell viability and has been reported recently to be present in 90S pre-ribosomal particles.	gene_phenotype
70327	1	333842	5	NULL	NULL	0	NULL	telomere	Chromosome	proximity of	is involved in		potentially			IMD1	GP	silencing of			NULL		0	NULL	NULL	NULL	gw70_genetics_173_2_1169_s_66	16582424	Thus, telomere proximity appears to be involved in the silencing of YAR073W/ IMD1.	gene_phenotype
70328	2	333842	5	NULL	NULL	0	NULL	YAR073W	NucleicAcid		is the locus name of					IMD1	GP				NULL		0	NULL	NULL	NULL	gw70_genetics_173_2_1169_s_66	16582424	Thus, telomere proximity appears to be involved in the silencing of YAR073W/ IMD1.	gene_phenotype
70331	1	333843	5	NULL	NULL	NULL	NULL	MD1	GP		is controlled by		potentially			TPE	Process	bona fide			NULL		NULL	NULL	NULL	NULL	gw70_genetics_173_2_1169_s_60	16582424	To examine whether YAR073W /MD1 was controlled by a  bona fide TPE, two different homeologous fragments from the middle of  Saccharomyces carlsbergensis chromosome  III, 7.0 and 8.4 kb in length, were inserted between YAR073W/ IMD1 and its proximal telomere and transcript levels were determined by quantitative RT - PCR as above.	gene_phenotype
70332	2	333843	5	NULL	NULL	0	NULL	YAR073W	NucleicAcid		is the locus name of					MD1	GP				NULL		0	NULL	NULL	NULL	gw70_genetics_173_2_1169_s_60	16582424	To examine whether YAR073W /MD1 was controlled by a  bona fide TPE, two different homeologous fragments from the middle of  Saccharomyces carlsbergensis chromosome  III, 7.0 and 8.4 kb in length, were inserted between YAR073W/ IMD1 and its proximal telomere and transcript levels were determined by quantitative RT - PCR as above.	gene_phenotype
70333	1	333844	5	NULL	NULL	0	NULL	YAR073W	NucleicAcid		is the locus name of					IMD1	GP				NULL		0	NULL	NULL	NULL	gw70_genetics_173_2_1169_s_23	16582424	In this report we demonstrate that the endmost chromosome  I ORF, YAR073W/ IMD1, is indeed silenced by its telomere, suggesting that telomeres play a role in silencing actual genes.	gene_phenotype
70335	2	333844	5	NULL	NULL	0	NULL	YAR073W	NucleicAcid		is a type of					chromosome I ORF	NucleicAcid	endmost			NULL		0	NULL	NULL	NULL	gw70_genetics_173_2_1169_s_23	16582424	In this report we demonstrate that the endmost chromosome  I ORF, YAR073W/ IMD1, is indeed silenced by its telomere, suggesting that telomeres play a role in silencing actual genes.	gene_phenotype
70337	3	333844	5	NULL	NULL	0	NULL	IMD1	GP		is silenced by					telomere	Chromosome				NULL		0	NULL	NULL	NULL	gw70_genetics_173_2_1169_s_23	16582424	In this report we demonstrate that the endmost chromosome  I ORF, YAR073W/ IMD1, is indeed silenced by its telomere, suggesting that telomeres play a role in silencing actual genes.	gene_phenotype
70338	4	333844	5	NULL	NULL	0	NULL	telomeres	Chromosome		plays a role in					genes	GP	silencing of;;actual			NULL		0	NULL	NULL	NULL	gw70_genetics_173_2_1169_s_23	16582424	In this report we demonstrate that the endmost chromosome  I ORF, YAR073W/ IMD1, is indeed silenced by its telomere, suggesting that telomeres play a role in silencing actual genes.	gene_phenotype
70339	1	333847	5	NULL	NULL	0	NULL	MJ0051 protein	GP	archaeal	activates					peptidyl-tRNA hydrolase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_35_37142_s_24	15210688	The SSO0175 and MJ0051 archaeal proteins, as well as the Ybl057c protein from  Saccharomyces cerevisiae (all from the PACE07 group), have been shown to have peptidyl-tRNA hydrolase activity and are thus involved in recycling peptidyl-tRNA molecules prematurely dissociated from the mRNA template ( ,  ).	gene_phenotype
70340	2	333847	5	NULL	NULL	0	NULL	SSO0175 protein	GP	archaeal	activates					peptidyl-tRNA hydrolase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_35_37142_s_24	15210688	The SSO0175 and MJ0051 archaeal proteins, as well as the Ybl057c protein from  Saccharomyces cerevisiae (all from the PACE07 group), have been shown to have peptidyl-tRNA hydrolase activity and are thus involved in recycling peptidyl-tRNA molecules prematurely dissociated from the mRNA template ( ,  ).	gene_phenotype
70341	3	333847	5	NULL	NULL	0	NULL	Ybl057c protein	GP	Saccharomyces cerevisiae	activates					peptidyl-tRNA hydrolase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_35_37142_s_24	15210688	The SSO0175 and MJ0051 archaeal proteins, as well as the Ybl057c protein from  Saccharomyces cerevisiae (all from the PACE07 group), have been shown to have peptidyl-tRNA hydrolase activity and are thus involved in recycling peptidyl-tRNA molecules prematurely dissociated from the mRNA template ( ,  ).	gene_phenotype
70342	4	333847	5	NULL	NULL	0	NULL	peptidyl-tRNA molecules	NucleicAcid		is dissociated from		prematurely			mRNA template	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_35_37142_s_24	15210688	The SSO0175 and MJ0051 archaeal proteins, as well as the Ybl057c protein from  Saccharomyces cerevisiae (all from the PACE07 group), have been shown to have peptidyl-tRNA hydrolase activity and are thus involved in recycling peptidyl-tRNA molecules prematurely dissociated from the mRNA template ( ,  ).	gene_phenotype
70343	5	333847	5	NULL	NULL	0	NULL	SSO0175 protein	GP	archaeal	recycles					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_35_37142_s_24	15210688	The SSO0175 and MJ0051 archaeal proteins, as well as the Ybl057c protein from  Saccharomyces cerevisiae (all from the PACE07 group), have been shown to have peptidyl-tRNA hydrolase activity and are thus involved in recycling peptidyl-tRNA molecules prematurely dissociated from the mRNA template ( ,  ).	gene_phenotype
70344	6	333847	5	NULL	NULL	0	NULL	MJ0051 protein	GP	archaeal	recycles					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_35_37142_s_24	15210688	The SSO0175 and MJ0051 archaeal proteins, as well as the Ybl057c protein from  Saccharomyces cerevisiae (all from the PACE07 group), have been shown to have peptidyl-tRNA hydrolase activity and are thus involved in recycling peptidyl-tRNA molecules prematurely dissociated from the mRNA template ( ,  ).	gene_phenotype
70345	7	333847	5	NULL	NULL	0	NULL	Ybl057c protein	GP	Saccharomyces cerevisiae	recycles					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_35_37142_s_24	15210688	The SSO0175 and MJ0051 archaeal proteins, as well as the Ybl057c protein from  Saccharomyces cerevisiae (all from the PACE07 group), have been shown to have peptidyl-tRNA hydrolase activity and are thus involved in recycling peptidyl-tRNA molecules prematurely dissociated from the mRNA template ( ,  ).	gene_phenotype
70346	1	333848	5	NULL	NULL	0	NULL	Msb2	GP		associate with		forced			Ybr062c	GP				NULL		0	NULL	NULL	NULL	gw70_genomeres_15_4_560_s_75	15805496	( B) Induction of the filamentous growth pathway occurs when Msb2 and Ybr062c are forced  to associate as leucine zipper fusions.	gene_phenotype
70347	2	333848	5	NULL	NULL	0	NULL	statement 1	Process		forms					leucine zipper fusions	GP				NULL		0	NULL	NULL	NULL	gw70_genomeres_15_4_560_s_75	15805496	( B) Induction of the filamentous growth pathway occurs when Msb2 and Ybr062c are forced  to associate as leucine zipper fusions.	gene_phenotype
70348	3	333848	5	NULL	NULL	0	NULL	statement 2	Process		induce					filamentous growth pathway	Process				NULL		0	NULL	NULL	NULL	gw70_genomeres_15_4_560_s_75	15805496	( B) Induction of the filamentous growth pathway occurs when Msb2 and Ybr062c are forced  to associate as leucine zipper fusions.	gene_phenotype
70349	1	333849	5	NULL	NULL	NULL	NULL	Ybr062c	NucleicAcid		interacts with		forced			Msb2	GP				NULL		NULL	NULL	NULL	NULL	gw70_genomeres_15_4_560_s_79	15805496	( C) Forced interaction between Ybr062c and Msb2 results in morphologies associated with  filamentous growth pathway hyperactivation.	gene_phenotype
70350	2	333849	5	NULL	NULL	0	NULL	statement 1	Process		is associated with					filamentous growth pathway	Process	hyperactivation of			NULL		0	NULL	NULL	NULL	gw70_genomeres_15_4_560_s_79	15805496	( C) Forced interaction between Ybr062c and Msb2 results in morphologies associated with  filamentous growth pathway hyperactivation.	gene_phenotype
70351	1	333850	5	NULL	NULL	0	NULL	Ybr062c	NucleicAcid		is not fused to					Fos	GP				NULL		0	NULL	NULL	NULL	gw70_genomeres_15_4_560_s_98	15805496	Overexpression of Ybr062c did not activate the filamentous growth pathway when not fused to Fos ( Fig. 3B); thus, it would not have been obtained in a high copy screen.	gene_phenotype
70352	2	333850	5	NULL	NULL	0	NULL	statement 1	Process	overexpression of	does not activate					filamentous growth pathway	Process				NULL		0	NULL	NULL	NULL	gw70_genomeres_15_4_560_s_98	15805496	Overexpression of Ybr062c did not activate the filamentous growth pathway when not fused to Fos ( Fig. 3B); thus, it would not have been obtained in a high copy screen.	gene_phenotype
70353	1	333851	5	NULL	NULL	0	NULL	YBR062c gene	GP	deletion of	does not disrupt					filamentous growth pathway	Process				NULL		0	NULL	NULL	NULL	gw70_genomeres_15_4_560_s_102	15805496	Deletion of the  YBR062c gene did not disrupt the filamentous growth pathway (data not shown), and as such, it would not have been recovered in a screen for loss-of-function mutations.	gene_phenotype
70354	1	333852	5	NULL	NULL	0	NULL	Ybr062c	NucleicAcid		does not play a role in		may;;primary			filamentous growth pathway	Process	activation of			NULL		0	NULL	NULL	NULL	gw70_genomeres_15_4_560_s_104	15805496	However, given the artificial nature of our screen, Ybr062c may not play a primary role in filamentous growth pathway activation but may influence another aspect of Msb2 function.	gene_phenotype
70355	2	333852	5	NULL	NULL	0	NULL	Ybr062c	NucleicAcid		influences					Msb2	GP	function of			NULL		0	NULL	NULL	NULL	gw70_genomeres_15_4_560_s_104	15805496	However, given the artificial nature of our screen, Ybr062c may not play a primary role in filamentous growth pathway activation but may influence another aspect of Msb2 function.	gene_phenotype
70358	1	333856	5	NULL	NULL	0	NULL	YFL030w protein	GP	yeast	activates					alanine:glyoxylate aminotransferase	GP				NULL		0	NULL	NULL	NULL	abs-batch0550-0559_biochimie_87_12_16226833_s_1	16226833	Crystal structure and confirmation of the alanine:glyoxylate aminotransferase activity of the YFL030w yeast protein..	gene_phenotype
70362	1	333862	5	NULL	NULL	0	NULL	YNR064c protein	GP		activates		low			epoxide hydrolase	GP				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_biochim-biophys-acta_1748_2_15769598_s_5	15769598	The YNR064c protein displayed low but reproducible epoxide hydrolase activity  with racemic phenanthrene 9,10-oxide and trans- or cis-stilbene oxide.	gene_phenotype
70364	2	333862	5	NULL	NULL	0	NULL	statement 1	Process		occurs with					phenanthrene 9,10-oxide	Chemical	racemic			NULL		0	NULL	NULL	NULL	abs-batch0680-0699_biochim-biophys-acta_1748_2_15769598_s_5	15769598	The YNR064c protein displayed low but reproducible epoxide hydrolase activity  with racemic phenanthrene 9,10-oxide and trans- or cis-stilbene oxide.	gene_phenotype
70365	3	333862	5	NULL	NULL	0	NULL	statement 1	Process		occurs with					trans- or cis-stilbene oxide	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_biochim-biophys-acta_1748_2_15769598_s_5	15769598	The YNR064c protein displayed low but reproducible epoxide hydrolase activity  with racemic phenanthrene 9,10-oxide and trans- or cis-stilbene oxide.	gene_phenotype
70368	1	333863	5	NULL	NULL	0	NULL	YA9E protein	GP		activates					Ap nA hydrolase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_13_8604_s_208	10085096	The gene encoding YA9E has recently been cloned and expressed, 4 and the protein has Ap nA hydrolase activity with Ap6A and Ap5A as the preferred substrates, but with some activity toward Ap4A, in contrast to YOR163w, which has no activity with this substrate.	gene_phenotype
70369	2	333863	5	NULL	NULL	0	NULL	Ap6A	GP		is a substrate of		preferred			Ap nA hydrolase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_13_8604_s_208	10085096	The gene encoding YA9E has recently been cloned and expressed, 4 and the protein has Ap nA hydrolase activity with Ap6A and Ap5A as the preferred substrates, but with some activity toward Ap4A, in contrast to YOR163w, which has no activity with this substrate.	gene_phenotype
70370	3	333863	5	NULL	NULL	0	NULL	Ap5A	GP		is a substrate of		preferred			Ap nA hydrolase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_13_8604_s_208	10085096	The gene encoding YA9E has recently been cloned and expressed, 4 and the protein has Ap nA hydrolase activity with Ap6A and Ap5A as the preferred substrates, but with some activity toward Ap4A, in contrast to YOR163w, which has no activity with this substrate.	gene_phenotype
70371	4	333863	5	NULL	NULL	0	NULL	Ap4A	GP		is a substrate of					Ap nA hydrolase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_13_8604_s_208	10085096	The gene encoding YA9E has recently been cloned and expressed, 4 and the protein has Ap nA hydrolase activity with Ap6A and Ap5A as the preferred substrates, but with some activity toward Ap4A, in contrast to YOR163w, which has no activity with this substrate.	gene_phenotype
70372	5	333863	5	NULL	NULL	0	NULL	YOR163w	NucleicAcid		has no activity with					Ap4A	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_13_8604_s_208	10085096	The gene encoding YA9E has recently been cloned and expressed, 4 and the protein has Ap nA hydrolase activity with Ap6A and Ap5A as the preferred substrates, but with some activity toward Ap4A, in contrast to YOR163w, which has no activity with this substrate.	gene_phenotype
70373	1	333864	5	NULL	NULL	0	NULL	YGL098w	NucleicAcid		codes for					SNARE-like protein	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_21_6_463_s_149	15116429	While this manuscript was in preparation, it was reported  that the  YGL098w codes for a product that is an ER-located SNARE-like protein involved in retrograde  transport of the vesicles (Dilcher  et al., [ 2003];	gene_phenotype
70374	2	333864	5	NULL	NULL	0	NULL	SNARE-like protein	GP		is located in					ER	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_21_6_463_s_149	15116429	While this manuscript was in preparation, it was reported  that the  YGL098w codes for a product that is an ER-located SNARE-like protein involved in retrograde  transport of the vesicles (Dilcher  et al., [ 2003];	gene_phenotype
70375	3	333864	5	NULL	NULL	0	NULL	SNARE-like protein	GP		is involved in					vesicle	CellComponent	retrograde transport of 			NULL		0	NULL	NULL	NULL	gw70_yeast_21_6_463_s_149	15116429	While this manuscript was in preparation, it was reported  that the  YGL098w codes for a product that is an ER-located SNARE-like protein involved in retrograde  transport of the vesicles (Dilcher  et al., [ 2003];	gene_phenotype
70376	1	333865	5	NULL	NULL	0	NULL	YGL098w gene	GP		is essential for					vegetative growth	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_yeast_16_4_10669874_s_7	10669874	Tetrad analysis of  heterozygous deletant strains revealed that YGL098w is an essential gene  for vegetative growth in three backgrounds, whereas the other five genes  are non-essential, although we have found some phenotypes in one of them.	gene_phenotype
70377	1	333866	5	NULL	NULL	0	NULL	YMR099cp	NucleicAcid		bind					hexose-6-phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_40_30175_s_131	16857670	The fact that sulfate ions often substitute for phosphate groups in protein structures ( ,  ) suggests that YMR099cp binds a hexose-6-phosphate and that it hence may have hexose-6-phosphate mutarotase (or 1-epimerase) activity.	gene_phenotype
70378	2	333866	5	NULL	NULL	0	NULL	YMR099cp	GP		activates					hexose-6-phosphate mutarotase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_40_30175_s_131	16857670	The fact that sulfate ions often substitute for phosphate groups in protein structures ( ,  ) suggests that YMR099cp binds a hexose-6-phosphate and that it hence may have hexose-6-phosphate mutarotase (or 1-epimerase) activity.	gene_phenotype
70379	3	333866	5	NULL	NULL	0	NULL	YMR099cp	NucleicAcid		activates					1-epimerase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_40_30175_s_131	16857670	The fact that sulfate ions often substitute for phosphate groups in protein structures ( ,  ) suggests that YMR099cp binds a hexose-6-phosphate and that it hence may have hexose-6-phosphate mutarotase (or 1-epimerase) activity.	gene_phenotype
70380	4	333866	5	NULL	NULL	0	NULL	sulfate ions	Chemical		substitute for					phosphate groups	Chemical				NULL	protein structures	0	NULL	NULL	NULL	gw70_jbiolchem_281_40_30175_s_131	16857670	The fact that sulfate ions often substitute for phosphate groups in protein structures ( ,  ) suggests that YMR099cp binds a hexose-6-phosphate and that it hence may have hexose-6-phosphate mutarotase (or 1-epimerase) activity.	gene_phenotype
70381	1	333867	5	NULL	NULL	0	NULL	YMR099cp protein	GP		activates					glucose-6-phosphate epimerase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_40_30175_s_142	16857670	In the second phase, faster generation of NAD(P)H reflecting higher velocity constant ( k+1) for the interconversion between glucose 6-phosphate anomers is obtained with increasing concentration of YMR099cp, demonstrating the glucose-6-phosphate epimerase activity of the protein ( Fig. 3 B,  inset).	gene_phenotype
70382	1	333869	5	NULL	NULL	0	NULL	YOR300W	NucleicAcid		is the locus name of					HUF1	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_162	15645503	HUF1  YOR300W May be involved in bipolar budding and bud site selection This study	gene_phenotype
70383	2	333869	5	NULL	NULL	0	NULL	HUF1	GP		is involved in					bipolar budding	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_162	15645503	HUF1  YOR300W May be involved in bipolar budding and bud site selection This study	gene_phenotype
70384	3	333869	5	NULL	NULL	0	NULL	HUF1	GP		is involved in					bud site selection 	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_162	15645503	HUF1  YOR300W May be involved in bipolar budding and bud site selection This study	gene_phenotype
70385	1	333870	5	NULL	NULL	0	NULL	bni1	GP	homozygous;;mutant	does not undergo					filamentous growth	Process				NULL	SLAD	0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_192	15645503	Homozygous  bni1 ,  bud2 ,  cap2 ,  ecm25 ,  gas1 ,  ilm1 ,  pea2 ,  sce66 ,  tpm1  and  YOR300W  1278 b mutants did not undergo filamentous growth on SLAD (Figure  3).	gene_phenotype
70386	2	333870	5	NULL	NULL	0	NULL	bud2	GP	homozygous;;mutant	does not undergo					filamentous growth	Process				NULL	SLAD	0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_192	15645503	Homozygous  bni1 ,  bud2 ,  cap2 ,  ecm25 ,  gas1 ,  ilm1 ,  pea2 ,  sce66 ,  tpm1  and  YOR300W  1278 b mutants did not undergo filamentous growth on SLAD (Figure  3).	gene_phenotype
70387	3	333870	5	NULL	NULL	0	NULL	cap2 	GP	homozygous;;mutant	does not undergo					filamentous growth	Process				NULL	SLAD	0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_192	15645503	Homozygous  bni1 ,  bud2 ,  cap2 ,  ecm25 ,  gas1 ,  ilm1 ,  pea2 ,  sce66 ,  tpm1  and  YOR300W  1278 b mutants did not undergo filamentous growth on SLAD (Figure  3).	gene_phenotype
70388	4	333870	5	NULL	NULL	0	NULL	ecm25	GP	homozygous;;mutant	does not undergo					filamentous growth	Process				NULL	SLAD	0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_192	15645503	Homozygous  bni1 ,  bud2 ,  cap2 ,  ecm25 ,  gas1 ,  ilm1 ,  pea2 ,  sce66 ,  tpm1  and  YOR300W  1278 b mutants did not undergo filamentous growth on SLAD (Figure  3).	gene_phenotype
70389	5	333870	5	NULL	NULL	0	NULL	gas1	GP	homozygous;;mutant	does not undergo					filamentous growth	Process				NULL	SLAD	0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_192	15645503	Homozygous  bni1 ,  bud2 ,  cap2 ,  ecm25 ,  gas1 ,  ilm1 ,  pea2 ,  sce66 ,  tpm1  and  YOR300W  1278 b mutants did not undergo filamentous growth on SLAD (Figure  3).	gene_phenotype
70390	6	333870	5	NULL	NULL	0	NULL	ilm1	GP	homozygous;;mutant	does not undergo					filamentous growth	Process				NULL	SLAD	0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_192	15645503	Homozygous  bni1 ,  bud2 ,  cap2 ,  ecm25 ,  gas1 ,  ilm1 ,  pea2 ,  sce66 ,  tpm1  and  YOR300W  1278 b mutants did not undergo filamentous growth on SLAD (Figure  3).	gene_phenotype
70391	7	333870	5	NULL	NULL	0	NULL	pea2	GP	homozygous;;mutant	does not undergo					filamentous growth	Process				NULL	SLAD	0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_192	15645503	Homozygous  bni1 ,  bud2 ,  cap2 ,  ecm25 ,  gas1 ,  ilm1 ,  pea2 ,  sce66 ,  tpm1  and  YOR300W  1278 b mutants did not undergo filamentous growth on SLAD (Figure  3).	gene_phenotype
70392	8	333870	5	NULL	NULL	0	NULL	sce66	GP	homozygous;;mutant	does not undergo					filamentous growth	Process				NULL	SLAD	0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_192	15645503	Homozygous  bni1 ,  bud2 ,  cap2 ,  ecm25 ,  gas1 ,  ilm1 ,  pea2 ,  sce66 ,  tpm1  and  YOR300W  1278 b mutants did not undergo filamentous growth on SLAD (Figure  3).	gene_phenotype
70393	9	333870	5	NULL	NULL	0	NULL	tpm1	GP	homozygous;;mutant	does not undergo					filamentous growth	Process				NULL	SLAD	0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_192	15645503	Homozygous  bni1 ,  bud2 ,  cap2 ,  ecm25 ,  gas1 ,  ilm1 ,  pea2 ,  sce66 ,  tpm1  and  YOR300W  1278 b mutants did not undergo filamentous growth on SLAD (Figure  3).	gene_phenotype
70394	10	333870	5	NULL	NULL	0	NULL	YOR300W	NucleicAcid	homozygous;;mutant	does not undergo					filamentous growth	Process				NULL	SLAD	0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_192	15645503	Homozygous  bni1 ,  bud2 ,  cap2 ,  ecm25 ,  gas1 ,  ilm1 ,  pea2 ,  sce66 ,  tpm1  and  YOR300W  1278 b mutants did not undergo filamentous growth on SLAD (Figure  3).	gene_phenotype
70527	1	333871	5	NULL	NULL	0	NULL	ABP1	GP		regulates					actin cytoskeleton	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_22_14_1143_s_31	16240455	The genes encode factors that regulate actin cytoskeleton/cell polarity ( ABP1, BNI1, BUD2, CAP2, PEA2, SPA2, TPM1 and YOR300W), cell wall structure and biosynthesis ( ECM25, GAS1 and  PRS3), protein secretion ( SEC66, RPL21A and  RPL34B) and mitochondria ( ILM1 and  UGO1).	gene_phenotype
70528	2	333871	5	NULL	NULL	0	NULL	ABP1	GP		regulates					cell polarity	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_14_1143_s_31	16240455	The genes encode factors that regulate actin cytoskeleton/cell polarity ( ABP1, BNI1, BUD2, CAP2, PEA2, SPA2, TPM1 and YOR300W), cell wall structure and biosynthesis ( ECM25, GAS1 and  PRS3), protein secretion ( SEC66, RPL21A and  RPL34B) and mitochondria ( ILM1 and  UGO1).	gene_phenotype
70529	3	333871	5	NULL	NULL	0	NULL	BNI1	GP		regulates					actin cytoskeleton	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_22_14_1143_s_31	16240455	The genes encode factors that regulate actin cytoskeleton/cell polarity ( ABP1, BNI1, BUD2, CAP2, PEA2, SPA2, TPM1 and YOR300W), cell wall structure and biosynthesis ( ECM25, GAS1 and  PRS3), protein secretion ( SEC66, RPL21A and  RPL34B) and mitochondria ( ILM1 and  UGO1).	gene_phenotype
70530	4	333871	5	NULL	NULL	0	NULL	BNI1	GP		regulates					cell polarity	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_14_1143_s_31	16240455	The genes encode factors that regulate actin cytoskeleton/cell polarity ( ABP1, BNI1, BUD2, CAP2, PEA2, SPA2, TPM1 and YOR300W), cell wall structure and biosynthesis ( ECM25, GAS1 and  PRS3), protein secretion ( SEC66, RPL21A and  RPL34B) and mitochondria ( ILM1 and  UGO1).	gene_phenotype
70531	5	333871	5	NULL	NULL	0	NULL	BUD2	GP		regulates					actin cytoskeleton	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_22_14_1143_s_31	16240455	The genes encode factors that regulate actin cytoskeleton/cell polarity ( ABP1, BNI1, BUD2, CAP2, PEA2, SPA2, TPM1 and YOR300W), cell wall structure and biosynthesis ( ECM25, GAS1 and  PRS3), protein secretion ( SEC66, RPL21A and  RPL34B) and mitochondria ( ILM1 and  UGO1).	gene_phenotype
70532	6	333871	5	NULL	NULL	0	NULL	BUD2	GP		regulates					cell polarity	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_14_1143_s_31	16240455	The genes encode factors that regulate actin cytoskeleton/cell polarity ( ABP1, BNI1, BUD2, CAP2, PEA2, SPA2, TPM1 and YOR300W), cell wall structure and biosynthesis ( ECM25, GAS1 and  PRS3), protein secretion ( SEC66, RPL21A and  RPL34B) and mitochondria ( ILM1 and  UGO1).	gene_phenotype
70533	7	333871	5	NULL	NULL	0	NULL	CAP2	GP		regulates					actin cytoskeleton	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_22_14_1143_s_31	16240455	The genes encode factors that regulate actin cytoskeleton/cell polarity ( ABP1, BNI1, BUD2, CAP2, PEA2, SPA2, TPM1 and YOR300W), cell wall structure and biosynthesis ( ECM25, GAS1 and  PRS3), protein secretion ( SEC66, RPL21A and  RPL34B) and mitochondria ( ILM1 and  UGO1).	gene_phenotype
70534	8	333871	5	NULL	NULL	0	NULL	CAP2	GP		regulates					cell polarity	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_14_1143_s_31	16240455	The genes encode factors that regulate actin cytoskeleton/cell polarity ( ABP1, BNI1, BUD2, CAP2, PEA2, SPA2, TPM1 and YOR300W), cell wall structure and biosynthesis ( ECM25, GAS1 and  PRS3), protein secretion ( SEC66, RPL21A and  RPL34B) and mitochondria ( ILM1 and  UGO1).	gene_phenotype
70535	9	333871	5	NULL	NULL	0	NULL	PEA2	GP		regulates					actin cytoskeleton	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_22_14_1143_s_31	16240455	The genes encode factors that regulate actin cytoskeleton/cell polarity ( ABP1, BNI1, BUD2, CAP2, PEA2, SPA2, TPM1 and YOR300W), cell wall structure and biosynthesis ( ECM25, GAS1 and  PRS3), protein secretion ( SEC66, RPL21A and  RPL34B) and mitochondria ( ILM1 and  UGO1).	gene_phenotype
70536	10	333871	5	NULL	NULL	0	NULL	PEA2	GP		regulates					cell polarity	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_14_1143_s_31	16240455	The genes encode factors that regulate actin cytoskeleton/cell polarity ( ABP1, BNI1, BUD2, CAP2, PEA2, SPA2, TPM1 and YOR300W), cell wall structure and biosynthesis ( ECM25, GAS1 and  PRS3), protein secretion ( SEC66, RPL21A and  RPL34B) and mitochondria ( ILM1 and  UGO1).	gene_phenotype
70537	11	333871	5	NULL	NULL	NULL	NULL	SPA2	GP		regulates					actin cytoskeleton	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_yeast_22_14_1143_s_31	16240455	The genes encode factors that regulate actin cytoskeleton/cell polarity ( ABP1, BNI1, BUD2, CAP2, PEA2, SPA2, TPM1 and YOR300W), cell wall structure and biosynthesis ( ECM25, GAS1 and  PRS3), protein secretion ( SEC66, RPL21A and  RPL34B) and mitochondria ( ILM1 and  UGO1).	gene_phenotype
70538	12	333871	5	NULL	NULL	0	NULL	SPA2	GP		regulates					cell polarity	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_14_1143_s_31	16240455	The genes encode factors that regulate actin cytoskeleton/cell polarity ( ABP1, BNI1, BUD2, CAP2, PEA2, SPA2, TPM1 and YOR300W), cell wall structure and biosynthesis ( ECM25, GAS1 and  PRS3), protein secretion ( SEC66, RPL21A and  RPL34B) and mitochondria ( ILM1 and  UGO1).	gene_phenotype
70539	13	333871	5	NULL	NULL	0	NULL	TPM1	GP		regulates					actin cytoskeleton	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_22_14_1143_s_31	16240455	The genes encode factors that regulate actin cytoskeleton/cell polarity ( ABP1, BNI1, BUD2, CAP2, PEA2, SPA2, TPM1 and YOR300W), cell wall structure and biosynthesis ( ECM25, GAS1 and  PRS3), protein secretion ( SEC66, RPL21A and  RPL34B) and mitochondria ( ILM1 and  UGO1).	gene_phenotype
70540	14	333871	5	NULL	NULL	0	NULL	TPM1	GP		regulates					cell polarity	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_14_1143_s_31	16240455	The genes encode factors that regulate actin cytoskeleton/cell polarity ( ABP1, BNI1, BUD2, CAP2, PEA2, SPA2, TPM1 and YOR300W), cell wall structure and biosynthesis ( ECM25, GAS1 and  PRS3), protein secretion ( SEC66, RPL21A and  RPL34B) and mitochondria ( ILM1 and  UGO1).	gene_phenotype
70541	15	333871	5	NULL	NULL	0	NULL	YOR300W	NucleicAcid		regulates					actin cytoskeleton	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_22_14_1143_s_31	16240455	The genes encode factors that regulate actin cytoskeleton/cell polarity ( ABP1, BNI1, BUD2, CAP2, PEA2, SPA2, TPM1 and YOR300W), cell wall structure and biosynthesis ( ECM25, GAS1 and  PRS3), protein secretion ( SEC66, RPL21A and  RPL34B) and mitochondria ( ILM1 and  UGO1).	gene_phenotype
70542	16	333871	5	NULL	NULL	0	NULL	YOR300W	NucleicAcid		regulates					cell polarity	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_14_1143_s_31	16240455	The genes encode factors that regulate actin cytoskeleton/cell polarity ( ABP1, BNI1, BUD2, CAP2, PEA2, SPA2, TPM1 and YOR300W), cell wall structure and biosynthesis ( ECM25, GAS1 and  PRS3), protein secretion ( SEC66, RPL21A and  RPL34B) and mitochondria ( ILM1 and  UGO1).	gene_phenotype
70543	17	333871	5	NULL	NULL	0	NULL	ECM25	GP		regulates					cell wall	CellComponent	structure of			NULL		0	NULL	NULL	NULL	gw70_yeast_22_14_1143_s_31	16240455	The genes encode factors that regulate actin cytoskeleton/cell polarity ( ABP1, BNI1, BUD2, CAP2, PEA2, SPA2, TPM1 and YOR300W), cell wall structure and biosynthesis ( ECM25, GAS1 and  PRS3), protein secretion ( SEC66, RPL21A and  RPL34B) and mitochondria ( ILM1 and  UGO1).	gene_phenotype
70544	18	333871	5	NULL	NULL	0	NULL	GAS1	GP		regulates					cell wall	CellComponent	structure of			NULL		0	NULL	NULL	NULL	gw70_yeast_22_14_1143_s_31	16240455	The genes encode factors that regulate actin cytoskeleton/cell polarity ( ABP1, BNI1, BUD2, CAP2, PEA2, SPA2, TPM1 and YOR300W), cell wall structure and biosynthesis ( ECM25, GAS1 and  PRS3), protein secretion ( SEC66, RPL21A and  RPL34B) and mitochondria ( ILM1 and  UGO1).	gene_phenotype
70545	19	333871	5	NULL	NULL	0	NULL	PRS3	GP		regulates					cell wall	CellComponent	structure of			NULL		0	NULL	NULL	NULL	gw70_yeast_22_14_1143_s_31	16240455	The genes encode factors that regulate actin cytoskeleton/cell polarity ( ABP1, BNI1, BUD2, CAP2, PEA2, SPA2, TPM1 and YOR300W), cell wall structure and biosynthesis ( ECM25, GAS1 and  PRS3), protein secretion ( SEC66, RPL21A and  RPL34B) and mitochondria ( ILM1 and  UGO1).	gene_phenotype
70546	20	333871	5	NULL	NULL	0	NULL	SEC66	GP		regulates					protein secretion	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_14_1143_s_31	16240455	The genes encode factors that regulate actin cytoskeleton/cell polarity ( ABP1, BNI1, BUD2, CAP2, PEA2, SPA2, TPM1 and YOR300W), cell wall structure and biosynthesis ( ECM25, GAS1 and  PRS3), protein secretion ( SEC66, RPL21A and  RPL34B) and mitochondria ( ILM1 and  UGO1).	gene_phenotype
70547	21	333871	5	NULL	NULL	0	NULL	RPL21A	GP		regulates					protein secretion	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_14_1143_s_31	16240455	The genes encode factors that regulate actin cytoskeleton/cell polarity ( ABP1, BNI1, BUD2, CAP2, PEA2, SPA2, TPM1 and YOR300W), cell wall structure and biosynthesis ( ECM25, GAS1 and  PRS3), protein secretion ( SEC66, RPL21A and  RPL34B) and mitochondria ( ILM1 and  UGO1).	gene_phenotype
70548	22	333871	5	NULL	NULL	0	NULL	RPL34B	GP		regulates					protein secretion	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_14_1143_s_31	16240455	The genes encode factors that regulate actin cytoskeleton/cell polarity ( ABP1, BNI1, BUD2, CAP2, PEA2, SPA2, TPM1 and YOR300W), cell wall structure and biosynthesis ( ECM25, GAS1 and  PRS3), protein secretion ( SEC66, RPL21A and  RPL34B) and mitochondria ( ILM1 and  UGO1).	gene_phenotype
70549	23	333871	5	NULL	NULL	0	NULL	ILM1	GP		regulates					mitochondria	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_22_14_1143_s_31	16240455	The genes encode factors that regulate actin cytoskeleton/cell polarity ( ABP1, BNI1, BUD2, CAP2, PEA2, SPA2, TPM1 and YOR300W), cell wall structure and biosynthesis ( ECM25, GAS1 and  PRS3), protein secretion ( SEC66, RPL21A and  RPL34B) and mitochondria ( ILM1 and  UGO1).	gene_phenotype
70550	24	333871	5	NULL	NULL	0	NULL	UGO1	GP		regulates					mitochondria	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_22_14_1143_s_31	16240455	The genes encode factors that regulate actin cytoskeleton/cell polarity ( ABP1, BNI1, BUD2, CAP2, PEA2, SPA2, TPM1 and YOR300W), cell wall structure and biosynthesis ( ECM25, GAS1 and  PRS3), protein secretion ( SEC66, RPL21A and  RPL34B) and mitochondria ( ILM1 and  UGO1).	gene_phenotype
70551	1	333872	5	NULL	NULL	0	NULL	ABP1	GP		regulates					actin cytoskeleton	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70552	2	333872	5	NULL	NULL	0	NULL	ABP1	GP		regulates					cell polarity	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70553	3	333872	5	NULL	NULL	0	NULL	CAP2	GP		regulates					actin cytoskeleton	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70554	4	333872	5	NULL	NULL	0	NULL	CAP2	GP		regulates					cell polarity	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70555	5	333872	5	NULL	NULL	0	NULL	HUF1	GP		regulates					actin cytoskeleton	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70556	6	333872	5	NULL	NULL	0	NULL	HUF1	GP		regulates					cell polarity	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70557	7	333872	5	NULL	NULL	0	NULL	YOR300W	NucleicAcid		is the locus name of					HUF1	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70558	8	333872	5	NULL	NULL	0	NULL	BNI1	GP		regulates					actin cytoskeleton	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70559	9	333872	5	NULL	NULL	0	NULL	BNI1	GP		regulates					cell polarity	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70560	10	333872	5	NULL	NULL	0	NULL	BUD2	GP		regulates					actin cytoskeleton	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70561	11	333872	5	NULL	NULL	0	NULL	BUD2	GP		regulates					cell polarity	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70562	12	333872	5	NULL	NULL	0	NULL	PEA2	GP		regulates					actin cytoskeleton	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70563	13	333872	5	NULL	NULL	0	NULL	PEA2	GP		regulates					cell polarity	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70564	14	333872	5	NULL	NULL	0	NULL	SPA2	GP		regulates					actin cytoskeleton	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70565	15	333872	5	NULL	NULL	0	NULL	SPA2	GP		regulates					cell polarity	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70566	16	333872	5	NULL	NULL	0	NULL	TPM1	GP		regulates					actin cytoskeleton	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70567	17	333872	5	NULL	NULL	0	NULL	TPM1	GP		regulates					cell polarity	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70568	18	333872	5	NULL	NULL	NULL	NULL	ECM25 gene	GP		is involved in		likely			cell wall	CellComponent	biosynthesis of			NULL		NULL	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70569	19	333872	5	NULL	NULL	0	NULL	GAS1 gene	GP		is involved in		likely			cell wall	CellComponent	biosynthesis of			NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70570	20	333872	5	NULL	NULL	NULL	NULL	PRS3 gene	GP		is involved in		likely			cell wall	CellComponent	biosynthesis of			NULL		NULL	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70571	21	333872	5	NULL	NULL	0	NULL	SEC66	GP		regulates		possibly			protein secretion	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70572	22	333872	5	NULL	NULL	0	NULL	RPL21A	GP		regulates		possibly			protein secretion	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70573	23	333872	5	NULL	NULL	0	NULL	RPL34B	GP		regulates		possibly			protein secretion	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70574	24	333872	5	NULL	NULL	0	NULL	IML1	GP		is involved in					mitochondria	CellComponent	normal function of			NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70575	25	333872	5	NULL	NULL	0	NULL	UGO1	GP		is involved in					mitochondria	CellComponent	normal function of			NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70576	26	333872	5	NULL	NULL	NULL	NULL	filamentous growth	Process	slow	is induced by					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70577	27	333872	5	NULL	NULL	NULL	NULL	ABP1 gene	GP		is required for					statement 26	Process				NULL		NULL	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70578	28	333872	5	NULL	NULL	NULL	NULL	ABP1 gene	GP		is required for					filamentous growth	Process	classic form of			NULL		NULL	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70579	29	333872	5	NULL	NULL	NULL	NULL	CAP2 gene	GP		is required for					statement 26	Process				NULL		NULL	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70580	30	333872	5	NULL	NULL	NULL	NULL	CAP2 gene	GP		is required for					filamentous growth	Process	classic form of			NULL		NULL	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70581	31	333872	5	NULL	NULL	NULL	NULL	HUF1 gene	GP		is required for					statement 26	Process				NULL		NULL	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70582	32	333872	5	NULL	NULL	NULL	NULL	HUF1 gene	GP		is required for					filamentous growth	Process	classic form of			NULL		NULL	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70583	33	333872	5	NULL	NULL	NULL	NULL	BNI1 gene	GP		is required for					statement 26	Process				NULL		NULL	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70584	34	333872	5	NULL	NULL	NULL	NULL	BNI1 gene	GP		is required for					filamentous growth	Process	classic form of			NULL		NULL	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70585	35	333872	5	NULL	NULL	NULL	NULL	BUD2 gene	GP		is required for					statement 26	Process				NULL		NULL	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70586	36	333872	5	NULL	NULL	NULL	NULL	BUD2 gene	GP		is required for					filamentous growth	Process	classic form of			NULL		NULL	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70587	37	333872	5	NULL	NULL	0	NULL	PEA2 gene	GP		is required for					statement 26	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70588	38	333872	5	NULL	NULL	0	NULL	PEA2 gene	GP		is required for					filamentous growth	Process	classic form of			NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70589	39	333872	5	NULL	NULL	0	NULL	SPA2 gene	GP		is required for					statement 26	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70590	40	333872	5	NULL	NULL	0	NULL	SPA2 gene	GP		is required for					filamentous growth	Process	classic form of			NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70591	41	333872	5	NULL	NULL	0	NULL	TPM1 gene	GP		is required for					statement 26	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70592	42	333872	5	NULL	NULL	0	NULL	TPM1 gene	GP		is required for					filamentous growth	Process	classic form of			NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70593	43	333872	5	NULL	NULL	0	NULL	ECM25 gene	GP		is required for					statement 26	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70594	44	333872	5	NULL	NULL	0	NULL	ECM25 gene	GP		is required for					filamentous growth	Process	classic form of			NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70595	45	333872	5	NULL	NULL	0	NULL	GAS1 gene	GP		is required for					statement 26	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70596	46	333872	5	NULL	NULL	0	NULL	GAS1 gene	GP		is required for					filamentous growth	Process	classic form of			NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70597	47	333872	5	NULL	NULL	0	NULL	PRS3 gene	GP		is required for					statement 26	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70598	48	333872	5	NULL	NULL	0	NULL	PRS3 gene	GP		is required for					filamentous growth	Process	classic form of			NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70599	49	333872	5	NULL	NULL	0	NULL	SEC66 gene	GP		is required for					statement 26	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70600	50	333872	5	NULL	NULL	0	NULL	SEC66 gene	GP		is required for					filamentous growth	Process	classic form of			NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70601	51	333872	5	NULL	NULL	0	NULL	RPL21A gene	GP		is required for					statement 26	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70602	52	333872	5	NULL	NULL	0	NULL	RPL21A gene	GP		is required for					filamentous growth	Process	classic form of			NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70603	53	333872	5	NULL	NULL	0	NULL	RPL34B gene	GP		is required for					statement 26	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70604	54	333872	5	NULL	NULL	0	NULL	RPL34B gene	GP		is required for					filamentous growth	Process	classic form of			NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70605	55	333872	5	NULL	NULL	0	NULL	IML1 gene	GP		is required for					statement 26	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70606	56	333872	5	NULL	NULL	0	NULL	IML1 gene	GP		is required for					filamentous growth	Process	classic form of			NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70607	57	333872	5	NULL	NULL	0	NULL	UGO1 gene	GP		is required for					statement 26	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70608	58	333872	5	NULL	NULL	0	NULL	UGO1 gene	GP		is required for					filamentous growth	Process	classic form of			NULL		0	NULL	NULL	NULL	gw70_yeast_22_2_79_s_3	15645503	We screened the BY yeast deletion strains and identified four classes of non-essential  genes that are required for both slowed DNA-induced filamentous growth and classic  forms of filamentous growth: (a) genes encoding regulators of the actin cytoskeleton  and cell polarity,  ABP1, CAP2 and  HUF1 (= YOR300W), in addition to the previously known  BNI1, BUD2, PEA2, SPA2 and  TPM1; (b) genes that are likely involved in cell wall biosynthesis,  ECM25, GAS1 and  PRS3; (c) genes encoding possible regulators of protein secretion,  SEC66, RPL21A and  RPL34B; (d) genes encoding factors for normal mitochondrial function,  IML1 and  UGO1.	gene_phenotype
70609	1	333873	5	NULL	NULL	NULL	NULL	sporulation	Process	defect in	is conferred by					cpr1delta/ cpr1delta	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_4_1_17_s_300	15643056	Thus, the sporulation defect conferred by a  cpr1delta/ cpr1delta mutation is suppressed by deletion of  SNT1,  SIF2,  YIL112W,  SET3, or  HOS2.	gene_phenotype
70610	2	333873	5	NULL	NULL	0	NULL	SNT1	GP	deletion of	suppress					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_1_17_s_300	15643056	Thus, the sporulation defect conferred by a  cpr1delta/ cpr1delta mutation is suppressed by deletion of  SNT1,  SIF2,  YIL112W,  SET3, or  HOS2.	gene_phenotype
70611	3	333873	5	NULL	NULL	0	NULL	SIF2	GP	deletion of	suppress					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_1_17_s_300	15643056	Thus, the sporulation defect conferred by a  cpr1delta/ cpr1delta mutation is suppressed by deletion of  SNT1,  SIF2,  YIL112W,  SET3, or  HOS2.	gene_phenotype
70612	4	333873	5	NULL	NULL	0	NULL	YIL112W	NucleicAcid	deletion of	suppress					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_1_17_s_300	15643056	Thus, the sporulation defect conferred by a  cpr1delta/ cpr1delta mutation is suppressed by deletion of  SNT1,  SIF2,  YIL112W,  SET3, or  HOS2.	gene_phenotype
70613	5	333873	5	NULL	NULL	0	NULL	SET3	GP	deletion of	suppress					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_1_17_s_300	15643056	Thus, the sporulation defect conferred by a  cpr1delta/ cpr1delta mutation is suppressed by deletion of  SNT1,  SIF2,  YIL112W,  SET3, or  HOS2.	gene_phenotype
70614	6	333873	5	NULL	NULL	0	NULL	HOS2	GP	deletion of	suppress					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_1_17_s_300	15643056	Thus, the sporulation defect conferred by a  cpr1delta/ cpr1delta mutation is suppressed by deletion of  SNT1,  SIF2,  YIL112W,  SET3, or  HOS2.	gene_phenotype
70615	1	333874	5	NULL	NULL	0	NULL	cpr1	GP	mutation of	effects		negatively			sporulation	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_1_17_s_303	15643056	Our data show that mutations in  SNT1,  SIF2,  YIL112W,  SET3, or  HOS2 counteract the negative effects of the  cpr1 mutation on sporulation, providing genetic evidence that the physical interactions observed between Cpr1 and the Set3 complex are functional.	gene_phenotype
70616	2	333874	5	NULL	NULL	0	NULL	SNT1	GP	mutant	counteract					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_1_17_s_303	15643056	Our data show that mutations in  SNT1,  SIF2,  YIL112W,  SET3, or  HOS2 counteract the negative effects of the  cpr1 mutation on sporulation, providing genetic evidence that the physical interactions observed between Cpr1 and the Set3 complex are functional.	gene_phenotype
70617	3	333874	5	NULL	NULL	0	NULL	SIF2	GP	mutant	counteract					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_1_17_s_303	15643056	Our data show that mutations in  SNT1,  SIF2,  YIL112W,  SET3, or  HOS2 counteract the negative effects of the  cpr1 mutation on sporulation, providing genetic evidence that the physical interactions observed between Cpr1 and the Set3 complex are functional.	gene_phenotype
70618	4	333874	5	NULL	NULL	0	NULL	YIL112W	NucleicAcid	mutant	counteract					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_1_17_s_303	15643056	Our data show that mutations in  SNT1,  SIF2,  YIL112W,  SET3, or  HOS2 counteract the negative effects of the  cpr1 mutation on sporulation, providing genetic evidence that the physical interactions observed between Cpr1 and the Set3 complex are functional.	gene_phenotype
70619	5	333874	5	NULL	NULL	0	NULL	SET3	GP	mutant	counteract					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_1_17_s_303	15643056	Our data show that mutations in  SNT1,  SIF2,  YIL112W,  SET3, or  HOS2 counteract the negative effects of the  cpr1 mutation on sporulation, providing genetic evidence that the physical interactions observed between Cpr1 and the Set3 complex are functional.	gene_phenotype
70620	6	333874	5	NULL	NULL	0	NULL	HOS2	GP	mutant	counteract					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_1_17_s_303	15643056	Our data show that mutations in  SNT1,  SIF2,  YIL112W,  SET3, or  HOS2 counteract the negative effects of the  cpr1 mutation on sporulation, providing genetic evidence that the physical interactions observed between Cpr1 and the Set3 complex are functional.	gene_phenotype
70621	7	333874	5	NULL	NULL	NULL	NULL	Cpr1	GP		interacts with		physically;;functionally			Set3 complex	GP				NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_4_1_17_s_303	15643056	Our data show that mutations in  SNT1,  SIF2,  YIL112W,  SET3, or  HOS2 counteract the negative effects of the  cpr1 mutation on sporulation, providing genetic evidence that the physical interactions observed between Cpr1 and the Set3 complex are functional.	gene_phenotype
70622	1	333875	5	NULL	NULL	0	NULL	SNT1	GP	mutant	enhances					sporulation	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_1_17_s_343	15643056	Another way to view this result is that deletion of  CPR1 partially counteracts the enhanced sporulation phenotype conferred by mutations in  SNT1,  SIF2,  YIL112W,  SET3, or  HOS2, indicating that cyclophilin A is required for full expression of this phenotype and therefore plays a positive role in meiosis regulation outside of its physical interactions with the Set3 complex.	gene_phenotype
70623	2	333875	5	NULL	NULL	0	NULL	SIF2	GP	mutant	enhances					sporulation	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_1_17_s_343	15643056	Another way to view this result is that deletion of  CPR1 partially counteracts the enhanced sporulation phenotype conferred by mutations in  SNT1,  SIF2,  YIL112W,  SET3, or  HOS2, indicating that cyclophilin A is required for full expression of this phenotype and therefore plays a positive role in meiosis regulation outside of its physical interactions with the Set3 complex.	gene_phenotype
70624	3	333875	5	NULL	NULL	0	NULL	YIL112W	NucleicAcid	mutant	enhances					sporulation	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_1_17_s_343	15643056	Another way to view this result is that deletion of  CPR1 partially counteracts the enhanced sporulation phenotype conferred by mutations in  SNT1,  SIF2,  YIL112W,  SET3, or  HOS2, indicating that cyclophilin A is required for full expression of this phenotype and therefore plays a positive role in meiosis regulation outside of its physical interactions with the Set3 complex.	gene_phenotype
70625	4	333875	5	NULL	NULL	0	NULL	SET3	GP	mutant	enhances					sporulation	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_1_17_s_343	15643056	Another way to view this result is that deletion of  CPR1 partially counteracts the enhanced sporulation phenotype conferred by mutations in  SNT1,  SIF2,  YIL112W,  SET3, or  HOS2, indicating that cyclophilin A is required for full expression of this phenotype and therefore plays a positive role in meiosis regulation outside of its physical interactions with the Set3 complex.	gene_phenotype
70626	5	333875	5	NULL	NULL	0	NULL	HOS2	GP	mutant	enhances					sporulation	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_1_17_s_343	15643056	Another way to view this result is that deletion of  CPR1 partially counteracts the enhanced sporulation phenotype conferred by mutations in  SNT1,  SIF2,  YIL112W,  SET3, or  HOS2, indicating that cyclophilin A is required for full expression of this phenotype and therefore plays a positive role in meiosis regulation outside of its physical interactions with the Set3 complex.	gene_phenotype
70627	6	333875	5	NULL	NULL	0	NULL	CPR1	GP	deletion of	counteract		partially			statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_1_17_s_343	15643056	Another way to view this result is that deletion of  CPR1 partially counteracts the enhanced sporulation phenotype conferred by mutations in  SNT1,  SIF2,  YIL112W,  SET3, or  HOS2, indicating that cyclophilin A is required for full expression of this phenotype and therefore plays a positive role in meiosis regulation outside of its physical interactions with the Set3 complex.	gene_phenotype
70628	7	333875	5	NULL	NULL	0	NULL	CPR1	GP	deletion of	counteract		partially			statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_1_17_s_343	15643056	Another way to view this result is that deletion of  CPR1 partially counteracts the enhanced sporulation phenotype conferred by mutations in  SNT1,  SIF2,  YIL112W,  SET3, or  HOS2, indicating that cyclophilin A is required for full expression of this phenotype and therefore plays a positive role in meiosis regulation outside of its physical interactions with the Set3 complex.	gene_phenotype
70629	8	333875	5	NULL	NULL	0	NULL	CPR1	GP	deletion of	counteract		partially			statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_1_17_s_343	15643056	Another way to view this result is that deletion of  CPR1 partially counteracts the enhanced sporulation phenotype conferred by mutations in  SNT1,  SIF2,  YIL112W,  SET3, or  HOS2, indicating that cyclophilin A is required for full expression of this phenotype and therefore plays a positive role in meiosis regulation outside of its physical interactions with the Set3 complex.	gene_phenotype
70630	9	333875	5	NULL	NULL	0	NULL	CPR1	GP	deletion of	counteract		partially			statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_1_17_s_343	15643056	Another way to view this result is that deletion of  CPR1 partially counteracts the enhanced sporulation phenotype conferred by mutations in  SNT1,  SIF2,  YIL112W,  SET3, or  HOS2, indicating that cyclophilin A is required for full expression of this phenotype and therefore plays a positive role in meiosis regulation outside of its physical interactions with the Set3 complex.	gene_phenotype
70631	10	333875	5	NULL	NULL	0	NULL	CPR1	GP	deletion of	counteract		partially			statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_1_17_s_343	15643056	Another way to view this result is that deletion of  CPR1 partially counteracts the enhanced sporulation phenotype conferred by mutations in  SNT1,  SIF2,  YIL112W,  SET3, or  HOS2, indicating that cyclophilin A is required for full expression of this phenotype and therefore plays a positive role in meiosis regulation outside of its physical interactions with the Set3 complex.	gene_phenotype
70632	11	333875	5	NULL	NULL	0	NULL	cyclophilin A	GP		is required for					sporulation	Process	full expression of			NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_1_17_s_343	15643056	Another way to view this result is that deletion of  CPR1 partially counteracts the enhanced sporulation phenotype conferred by mutations in  SNT1,  SIF2,  YIL112W,  SET3, or  HOS2, indicating that cyclophilin A is required for full expression of this phenotype and therefore plays a positive role in meiosis regulation outside of its physical interactions with the Set3 complex.	gene_phenotype
70633	12	333875	5	NULL	NULL	NULL	NULL	CPR1	GP		regulates		positive			meiosis	Process				NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_4_1_17_s_343	15643056	Another way to view this result is that deletion of  CPR1 partially counteracts the enhanced sporulation phenotype conferred by mutations in  SNT1,  SIF2,  YIL112W,  SET3, or  HOS2, indicating that cyclophilin A is required for full expression of this phenotype and therefore plays a positive role in meiosis regulation outside of its physical interactions with the Set3 complex.	gene_phenotype
70634	13	333875	5	NULL	NULL	0	NULL	CPR1	GP		interacts with		physically			Set3 complex	GP				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_1_17_s_343	15643056	Another way to view this result is that deletion of  CPR1 partially counteracts the enhanced sporulation phenotype conferred by mutations in  SNT1,  SIF2,  YIL112W,  SET3, or  HOS2, indicating that cyclophilin A is required for full expression of this phenotype and therefore plays a positive role in meiosis regulation outside of its physical interactions with the Set3 complex.	gene_phenotype
70635	1	333877	5	NULL	NULL	0	NULL	YBR159w protein	GP		activates					3-ketoacyl-CoA reductase					NULL	yeast microsomes	0	NULL	NULL	NULL	gw70_jbiolchem_278_9_7335_s_43	12482854	The  YBR159w gene encoded the protein that was responsible for the majority of the 3-ketoacyl-CoA reductase activity in yeast microsomes ( ).	gene_phenotype
70636	1	333879	5	NULL	NULL	0	NULL	Ayr1p	GP		activates					3-ketoreductase	GP	residual			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_38_35440_s_10	12087109	By disrupting the orthologs of  Ybr159w in the  ybr159delta mutant we found that the  ybr159deltaayr1delta double mutant was inviable, suggesting that Ayr1p is responsible for the residual 3-ketoreductase activity.	gene_phenotype
70637	1	333883	5	NULL	NULL	0	NULL	YBR159w gene	GP	deletion of	slows					growth	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_38_35440_s_123	12087109	Deletion of the YBR159w Gene Causes Slow Growth, Suppression of the Ca2+-sensitive Phenotype Associated with the csg2delta Mutation, and Synthetic Lethality with the elo2delta Mutation-- The Ybr159p protein was previously shown to be required for C2 elongation of polyunsaturated fatty acids mediated by heterologous expression of a  C. elegans polyunsaturated fatty acid-elongating activity F56H11.4 activity in  S. cerevisiae ( 11).	gene_phenotype
70638	2	333883	5	NULL	NULL	0	NULL	Ca2+-sensitive phenotype	PhysicalPhenomenon	suppression of	is associated with					csg2delta	GP	mutant			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_38_35440_s_123	12087109	Deletion of the YBR159w Gene Causes Slow Growth, Suppression of the Ca2+-sensitive Phenotype Associated with the csg2delta Mutation, and Synthetic Lethality with the elo2delta Mutation-- The Ybr159p protein was previously shown to be required for C2 elongation of polyunsaturated fatty acids mediated by heterologous expression of a  C. elegans polyunsaturated fatty acid-elongating activity F56H11.4 activity in  S. cerevisiae ( 11).	gene_phenotype
70639	3	333883	5	NULL	NULL	0	NULL	lethality	Process	synthetic	is associated with					elo2delta	GP	mutant			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_38_35440_s_123	12087109	Deletion of the YBR159w Gene Causes Slow Growth, Suppression of the Ca2+-sensitive Phenotype Associated with the csg2delta Mutation, and Synthetic Lethality with the elo2delta Mutation-- The Ybr159p protein was previously shown to be required for C2 elongation of polyunsaturated fatty acids mediated by heterologous expression of a  C. elegans polyunsaturated fatty acid-elongating activity F56H11.4 activity in  S. cerevisiae ( 11).	gene_phenotype
70640	4	333883	5	NULL	NULL	0	NULL	polyunsaturated fatty acids	Chemical	C2 elongation of 	is mediated by					F56H11.4 activity	GP	C. elegans			NULL	S. cerevisiae	0	NULL	NULL	NULL	gw60_jbiolchem_277_38_35440_s_123	12087109	Deletion of the YBR159w Gene Causes Slow Growth, Suppression of the Ca2+-sensitive Phenotype Associated with the csg2delta Mutation, and Synthetic Lethality with the elo2delta Mutation-- The Ybr159p protein was previously shown to be required for C2 elongation of polyunsaturated fatty acids mediated by heterologous expression of a  C. elegans polyunsaturated fatty acid-elongating activity F56H11.4 activity in  S. cerevisiae ( 11).	gene_phenotype
70641	5	333883	5	NULL	NULL	0	NULL	Ybr159p protein	GP		is required for					statement 1	Process				NULL	S.cerevisiae	0	NULL	NULL	NULL	gw60_jbiolchem_277_38_35440_s_123	12087109	Deletion of the YBR159w Gene Causes Slow Growth, Suppression of the Ca2+-sensitive Phenotype Associated with the csg2delta Mutation, and Synthetic Lethality with the elo2delta Mutation-- The Ybr159p protein was previously shown to be required for C2 elongation of polyunsaturated fatty acids mediated by heterologous expression of a  C. elegans polyunsaturated fatty acid-elongating activity F56H11.4 activity in  S. cerevisiae ( 11).	gene_phenotype
70642	6	333883	5	NULL	NULL	0	NULL	F56H11.4	GP		is a synonym of					polyunsaturated fatty acid-elongating	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_38_35440_s_123	12087109	Deletion of the YBR159w Gene Causes Slow Growth, Suppression of the Ca2+-sensitive Phenotype Associated with the csg2delta Mutation, and Synthetic Lethality with the elo2delta Mutation-- The Ybr159p protein was previously shown to be required for C2 elongation of polyunsaturated fatty acids mediated by heterologous expression of a  C. elegans polyunsaturated fatty acid-elongating activity F56H11.4 activity in  S. cerevisiae ( 11).	gene_phenotype
70647	1	333884	5	NULL	NULL	0	NULL	snoRNAs	NucleicAcid		is					small nucleolar RNAs	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_pnas_103_32_11898_s_18	16882719	Similarly, many small nucleolar RNAs (snoRNAs) depend on the exosome during their maturation ( ,  ), and deletion of Rrp6p in yeast also leads to accumulation of extended forms of both polycistronic snoRNAs ( ) and the independently transcribed snoRNAs, such as snR33 and snR40 ( ).	gene_phenotype
70648	2	333884	5	NULL	NULL	NULL	NULL	snoRNAs	NucleicAcid		depends on					snoRNAs	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_32_11898_s_18	16882719	Similarly, many small nucleolar RNAs (snoRNAs) depend on the exosome during their maturation ( ,  ), and deletion of Rrp6p in yeast also leads to accumulation of extended forms of both polycistronic snoRNAs ( ) and the independently transcribed snoRNAs, such as snR33 and snR40 ( ).	gene_phenotype
70755	3	333884	5	NULL	NULL	0	NULL	statement 2	Process		occurs during					snoRNAs	NucleicAcid	maturation of			NULL		0	NULL	NULL	NULL	gw70_pnas_103_32_11898_s_18	16882719	Similarly, many small nucleolar RNAs (snoRNAs) depend on the exosome during their maturation ( ,  ), and deletion of Rrp6p in yeast also leads to accumulation of extended forms of both polycistronic snoRNAs ( ) and the independently transcribed snoRNAs, such as snR33 and snR40 ( ).	gene_phenotype
70756	4	333884	5	NULL	NULL	NULL	NULL	Rrp6p	GP	deletion of	accumulates					snoRNAs	NucleicAcid	extended forms of;;polycistronic			NULL	yeast	NULL	NULL	NULL	NULL	gw70_pnas_103_32_11898_s_18	16882719	Similarly, many small nucleolar RNAs (snoRNAs) depend on the exosome during their maturation ( ,  ), and deletion of Rrp6p in yeast also leads to accumulation of extended forms of both polycistronic snoRNAs ( ) and the independently transcribed snoRNAs, such as snR33 and snR40 ( ).	gene_phenotype
70757	5	333884	5	NULL	NULL	0	NULL	Rrp6p	GP	deletion of	accumulates					snR33As	NucleicAcid				NULL	yeast	0	NULL	NULL	NULL	gw70_pnas_103_32_11898_s_18	16882719	Similarly, many small nucleolar RNAs (snoRNAs) depend on the exosome during their maturation ( ,  ), and deletion of Rrp6p in yeast also leads to accumulation of extended forms of both polycistronic snoRNAs ( ) and the independently transcribed snoRNAs, such as snR33 and snR40 ( ).	gene_phenotype
70758	6	333884	5	NULL	NULL	0	NULL	Rrp6p	GP	deletion of	accumulates					snR40	NucleicAcid				NULL	yeast	0	NULL	NULL	NULL	gw70_pnas_103_32_11898_s_18	16882719	Similarly, many small nucleolar RNAs (snoRNAs) depend on the exosome during their maturation ( ,  ), and deletion of Rrp6p in yeast also leads to accumulation of extended forms of both polycistronic snoRNAs ( ) and the independently transcribed snoRNAs, such as snR33 and snR40 ( ).	gene_phenotype
70759	7	333884	5	NULL	NULL	0	NULL	snR33	NucleicAcid		is a type of					independently transcribed snoRNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_pnas_103_32_11898_s_18	16882719	Similarly, many small nucleolar RNAs (snoRNAs) depend on the exosome during their maturation ( ,  ), and deletion of Rrp6p in yeast also leads to accumulation of extended forms of both polycistronic snoRNAs ( ) and the independently transcribed snoRNAs, such as snR33 and snR40 ( ).	gene_phenotype
70760	8	333884	5	NULL	NULL	0	NULL	snR40	NucleicAcid		is a type of					independently transcribed snoRNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_pnas_103_32_11898_s_18	16882719	Similarly, many small nucleolar RNAs (snoRNAs) depend on the exosome during their maturation ( ,  ), and deletion of Rrp6p in yeast also leads to accumulation of extended forms of both polycistronic snoRNAs ( ) and the independently transcribed snoRNAs, such as snR33 and snR40 ( ).	gene_phenotype
70761	1	333885	5	NULL	NULL	0	NULL	YKR079C gene	GP		is indispensable for					yeast	Cell	viability of			NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_31_9_2272_s_177	12711671	The  YKR079C gene has been shown to be indispensable for yeast viability ( 1), suggesting that the yeast genome may have only one gene that encodes an enzyme responsible for correctly removing 3' trailers from pre-tRNAs.	gene_phenotype
70762	1	333886	5	NULL	NULL	0	NULL	ELAC1	GP	human	activates		possibly			tRNA 3'	NucleicAcid	processing of			NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_31_9_2272_s_136	12711671	To examine whether ELAC1 has also the tRNA 3' processing activity as ELAC2-deltaN, we cloned a human cDNA encoding ELAC1 into the plasmid pGEX-4T-3, and expressed and purified the GST - ELAC1 fusion protein as described for GST - YKR079C (Fig.  2).	gene_phenotype
70763	2	333886	5	NULL	NULL	0	NULL	ELAC2-deltaN	GP		activates					tRNA 3'	NucleicAcid	processing of			NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_31_9_2272_s_136	12711671	To examine whether ELAC1 has also the tRNA 3' processing activity as ELAC2-deltaN, we cloned a human cDNA encoding ELAC1 into the plasmid pGEX-4T-3, and expressed and purified the GST - ELAC1 fusion protein as described for GST - YKR079C (Fig.  2).	gene_phenotype
70764	1	333888	5	NULL	NULL	0	NULL	MAPK pathway	Process		is regulated by					PKC	GP				NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_49	10657304	MPK1,  MLP1,  RLM1, and  YLR194C were induced under conditions that activate the PKC-regulated MAPK pathway;  KSS1,  YLRO42C,  PGU1, and  SVS1 are potential filamentous growth genes induced preferentially by Kss1p signaling.	gene_phenotype
70765	2	333888	5	NULL	NULL	0	NULL	KSS1	GP		is induced by		preferentially			Kss1p signaling	Process				NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_49	10657304	MPK1,  MLP1,  RLM1, and  YLR194C were induced under conditions that activate the PKC-regulated MAPK pathway;  KSS1,  YLRO42C,  PGU1, and  SVS1 are potential filamentous growth genes induced preferentially by Kss1p signaling.	gene_phenotype
70768	3	333888	5	NULL	NULL	0	NULL	YLRO42C	NucleicAcid		is induced by		preferentially			Kss1p signaling	Process				NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_49	10657304	MPK1,  MLP1,  RLM1, and  YLR194C were induced under conditions that activate the PKC-regulated MAPK pathway;  KSS1,  YLRO42C,  PGU1, and  SVS1 are potential filamentous growth genes induced preferentially by Kss1p signaling.	gene_phenotype
70769	4	333888	5	NULL	NULL	0	NULL	PGU1	GP		is induced by		preferentially			Kss1p signaling	Process				NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_49	10657304	MPK1,  MLP1,  RLM1, and  YLR194C were induced under conditions that activate the PKC-regulated MAPK pathway;  KSS1,  YLRO42C,  PGU1, and  SVS1 are potential filamentous growth genes induced preferentially by Kss1p signaling.	gene_phenotype
70770	5	333888	5	NULL	NULL	0	NULL	SVS1	GP		is induced by		preferentially			Kss1p signaling	Process				NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_49	10657304	MPK1,  MLP1,  RLM1, and  YLR194C were induced under conditions that activate the PKC-regulated MAPK pathway;  KSS1,  YLRO42C,  PGU1, and  SVS1 are potential filamentous growth genes induced preferentially by Kss1p signaling.	gene_phenotype
70773	6	333888	5	NULL	NULL	0	NULL	KSS1	GP		is a type of					filamentous growth gene	GP	potential			NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_49	10657304	MPK1,  MLP1,  RLM1, and  YLR194C were induced under conditions that activate the PKC-regulated MAPK pathway;  KSS1,  YLRO42C,  PGU1, and  SVS1 are potential filamentous growth genes induced preferentially by Kss1p signaling.	gene_phenotype
70774	7	333888	5	NULL	NULL	0	NULL	YLRO42C	GP		is a type of					filamentous growth gene	GP	potential			NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_49	10657304	MPK1,  MLP1,  RLM1, and  YLR194C were induced under conditions that activate the PKC-regulated MAPK pathway;  KSS1,  YLRO42C,  PGU1, and  SVS1 are potential filamentous growth genes induced preferentially by Kss1p signaling.	gene_phenotype
70775	8	333888	5	NULL	NULL	0	NULL	PGU1	GP		is a type of					filamentous growth gene	GP	potential			NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_49	10657304	MPK1,  MLP1,  RLM1, and  YLR194C were induced under conditions that activate the PKC-regulated MAPK pathway;  KSS1,  YLRO42C,  PGU1, and  SVS1 are potential filamentous growth genes induced preferentially by Kss1p signaling.	gene_phenotype
70776	9	333888	5	NULL	NULL	0	NULL	SVS1	GP		is a type of					filamentous growth gene	GP	potential			NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_49	10657304	MPK1,  MLP1,  RLM1, and  YLR194C were induced under conditions that activate the PKC-regulated MAPK pathway;  KSS1,  YLRO42C,  PGU1, and  SVS1 are potential filamentous growth genes induced preferentially by Kss1p signaling.	gene_phenotype
70777	1	333890	5	NULL	NULL	0	NULL	Prp40p	GP		contains					NESs	AminoAcid	redundant			NULL		0	NULL	NULL	NULL	gw70_genetics_166_1_53_s_11	15020406	Although we do not expect that yeast snRNPs undergo compartmentalized biogenesis like their metazoan counterparts, our results suggest that Prp40p and Ynl187wp contain redundant NESs that aid in an important, Crm1p-mediated nuclear export event.	gene_phenotype
70778	2	333890	5	NULL	NULL	0	NULL	Ynl187wp	NucleicAcid		contains					NESs	AminoAcid	redundant			NULL		0	NULL	NULL	NULL	gw70_genetics_166_1_53_s_11	15020406	Although we do not expect that yeast snRNPs undergo compartmentalized biogenesis like their metazoan counterparts, our results suggest that Prp40p and Ynl187wp contain redundant NESs that aid in an important, Crm1p-mediated nuclear export event.	gene_phenotype
70779	3	333890	5	NULL	NULL	0	NULL	nuclear export	Process		is mediated by					Crm1p	GP				NULL		0	NULL	NULL	NULL	gw70_genetics_166_1_53_s_11	15020406	Although we do not expect that yeast snRNPs undergo compartmentalized biogenesis like their metazoan counterparts, our results suggest that Prp40p and Ynl187wp contain redundant NESs that aid in an important, Crm1p-mediated nuclear export event.	gene_phenotype
70780	4	333890	5	NULL	NULL	0	NULL	NESs	AminoAcid	redundant	aid in					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_genetics_166_1_53_s_11	15020406	Although we do not expect that yeast snRNPs undergo compartmentalized biogenesis like their metazoan counterparts, our results suggest that Prp40p and Ynl187wp contain redundant NESs that aid in an important, Crm1p-mediated nuclear export event.	gene_phenotype
70781	1	333891	5	NULL	NULL	0	NULL	nuclear export	Process		is mediated by					Crm1p	GP				NULL		0	NULL	NULL	NULL	gw70_genetics_166_1_53_s_408	15020406	Together our results suggest a model in which Prp40p and Ynl187wp contain redundant, functional leucine-rich nuclear export signals that aid in a Crm1p-mediated nuclear export event.	gene_phenotype
70782	2	333891	5	NULL	NULL	0	NULL	Prp40p	GP		contains					leucine-rich nuclear export signals	AminoAcid	redundant;;functional			NULL		0	NULL	NULL	NULL	gw70_genetics_166_1_53_s_408	15020406	Together our results suggest a model in which Prp40p and Ynl187wp contain redundant, functional leucine-rich nuclear export signals that aid in a Crm1p-mediated nuclear export event.	gene_phenotype
70783	3	333891	5	NULL	NULL	0	NULL	Ynl187wp	NucleicAcid		contains					leucine-rich nuclear export signals	AminoAcid	redundant;;functional			NULL		0	NULL	NULL	NULL	gw70_genetics_166_1_53_s_408	15020406	Together our results suggest a model in which Prp40p and Ynl187wp contain redundant, functional leucine-rich nuclear export signals that aid in a Crm1p-mediated nuclear export event.	gene_phenotype
70784	4	333891	5	NULL	NULL	0	NULL	leucine-rich nuclear export signals	AminoAcid	redundant;;functional	aid in					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_genetics_166_1_53_s_408	15020406	Together our results suggest a model in which Prp40p and Ynl187wp contain redundant, functional leucine-rich nuclear export signals that aid in a Crm1p-mediated nuclear export event.	gene_phenotype
70785	1	333892	5	NULL	NULL	NULL	NULL	NESs	AminoAcid		is mutated in					prp40delta	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw70_genetics_166_1_53_s_357	15020406	Mutation of both NESs ( prp40delta 2 ynl187w-slf) would thus result in the loss of nuclear export of a complex.	gene_phenotype
70786	2	333892	5	NULL	NULL	NULL	NULL	NESs	AminoAcid		is mutated in					ynl187w-slf	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw70_genetics_166_1_53_s_357	15020406	Mutation of both NESs ( prp40delta 2 ynl187w-slf) would thus result in the loss of nuclear export of a complex.	gene_phenotype
70787	3	333892	5	NULL	NULL	NULL	NULL	statement 1	Process		results in					nuclear export	Process	loss of			NULL		NULL	NULL	NULL	NULL	gw70_genetics_166_1_53_s_357	15020406	Mutation of both NESs ( prp40delta 2 ynl187w-slf) would thus result in the loss of nuclear export of a complex.	gene_phenotype
70788	4	333892	5	NULL	NULL	NULL	NULL	statement 2	Process		results in					nuclear export	Process	loss of			NULL		NULL	NULL	NULL	NULL	gw70_genetics_166_1_53_s_357	15020406	Mutation of both NESs ( prp40delta 2 ynl187w-slf) would thus result in the loss of nuclear export of a complex.	gene_phenotype
70789	1	333893	5	NULL	NULL	0	NULL	SUL1 gene	GP		is involved in					sulphate	Chemical	uptake of			NULL		0	NULL	NULL	NULL	gw70_yeast_19_6_475_s_42	11921096	Three genes are involved in sulphate uptake:  SUL1 and  SUL2 encoding high-affinity sulphate transport proteins, and  SUL3 encoding a factor involved in the transcriptional regulation of  SUL2 (Cherest  et al., [ 1997]).	gene_phenotype
70790	2	333893	5	NULL	NULL	0	NULL	SUL2 gene	GP		is involved in					sulphate	Chemical	uptake of			NULL		0	NULL	NULL	NULL	gw70_yeast_19_6_475_s_42	11921096	Three genes are involved in sulphate uptake:  SUL1 and  SUL2 encoding high-affinity sulphate transport proteins, and  SUL3 encoding a factor involved in the transcriptional regulation of  SUL2 (Cherest  et al., [ 1997]).	gene_phenotype
70791	3	333893	5	NULL	NULL	0	NULL	SUL3 gene	GP		is involved in					sulphate	Chemical	uptake of			NULL		0	NULL	NULL	NULL	gw70_yeast_19_6_475_s_42	11921096	Three genes are involved in sulphate uptake:  SUL1 and  SUL2 encoding high-affinity sulphate transport proteins, and  SUL3 encoding a factor involved in the transcriptional regulation of  SUL2 (Cherest  et al., [ 1997]).	gene_phenotype
70792	4	333893	5	NULL	NULL	0	NULL	SUL1 gene	GP		encodes for					sulphate transport proteins	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_19_6_475_s_42	11921096	Three genes are involved in sulphate uptake:  SUL1 and  SUL2 encoding high-affinity sulphate transport proteins, and  SUL3 encoding a factor involved in the transcriptional regulation of  SUL2 (Cherest  et al., [ 1997]).	gene_phenotype
70793	5	333893	5	NULL	NULL	NULL	NULL	SUL2 gene	GP		encodes for					sulphate transport proteins	GP				NULL		NULL	NULL	NULL	NULL	gw70_yeast_19_6_475_s_42	11921096	Three genes are involved in sulphate uptake:  SUL1 and  SUL2 encoding high-affinity sulphate transport proteins, and  SUL3 encoding a factor involved in the transcriptional regulation of  SUL2 (Cherest  et al., [ 1997]).	gene_phenotype
70794	6	333893	5	NULL	NULL	0	NULL	SUL3 gene	GP		is involved in					SUL2	GP	transcriptional regulation of			NULL		0	NULL	NULL	NULL	gw70_yeast_19_6_475_s_42	11921096	Three genes are involved in sulphate uptake:  SUL1 and  SUL2 encoding high-affinity sulphate transport proteins, and  SUL3 encoding a factor involved in the transcriptional regulation of  SUL2 (Cherest  et al., [ 1997]).	gene_phenotype
70795	1	333894	5	NULL	NULL	0	NULL	YOL002c protein	GP		accumulates					polyphosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_22_19609_s_231	11916977	The YOL002c Protein Is Involved in Polyphosphate Accumulation and in Regulation of Acid Phosphatase Activity-- Polyphosphate is a linear polymer of up to hundreds of Pi residues linked by phosphoanhydride bonds.	gene_phenotype
70796	2	333894	5	NULL	NULL	0	NULL	YOL002c protein	GP		regulates					acid phosphatase activity	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_22_19609_s_231	11916977	The YOL002c Protein Is Involved in Polyphosphate Accumulation and in Regulation of Acid Phosphatase Activity-- Polyphosphate is a linear polymer of up to hundreds of Pi residues linked by phosphoanhydride bonds.	gene_phenotype
70797	3	333894	5	NULL	NULL	0	NULL	Pi residues	Chemical	hundreds of	is linked by					phosphoanhydride bonds	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_22_19609_s_231	11916977	The YOL002c Protein Is Involved in Polyphosphate Accumulation and in Regulation of Acid Phosphatase Activity-- Polyphosphate is a linear polymer of up to hundreds of Pi residues linked by phosphoanhydride bonds.	gene_phenotype
70798	4	333894	5	NULL	NULL	0	NULL	polyphosphate	Chemical		is a polymer of		linear			statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_22_19609_s_231	11916977	The YOL002c Protein Is Involved in Polyphosphate Accumulation and in Regulation of Acid Phosphatase Activity-- Polyphosphate is a linear polymer of up to hundreds of Pi residues linked by phosphoanhydride bonds.	gene_phenotype
70799	1	333895	5	NULL	NULL	0	NULL	YOL002c	NucleicAcid	deletion of	derepress					acid phosphatase activity	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_22_19609_s_284	11916977	Because deletion of  YOL002c results in a strain that is incapable of derepressing acid phosphatase activity ( i.e. constitutive  PHO5 expression), it is possible that this protein plays a similar role to that of Pho23p.	gene_phenotype
70800	2	333895	5	NULL	NULL	0	NULL	YOL002c protein	GP	role of	is similar to					Pho23p	GP	role of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_22_19609_s_284	11916977	Because deletion of  YOL002c results in a strain that is incapable of derepressing acid phosphatase activity ( i.e. constitutive  PHO5 expression), it is possible that this protein plays a similar role to that of Pho23p.	gene_phenotype
70801	2	333896	5	NULL	NULL	0	NULL	Yjl103c protein	GP		interacts with					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_7_553_s_261	16710832	The Yjl103c protein interacts (Hazbun  et al., [ 2003]) with the products of genes involved in nuclear positioning ( p < 5.0 x 10-3).	gene_phenotype
70802	1	333896	5	NULL	NULL	0	NULL	gene products	GP		is involved in					nucleus	CellComponent	positioning of			NULL		0	NULL	NULL	NULL	gw70_yeast_23_7_553_s_261	16710832	The Yjl103c protein interacts (Hazbun  et al., [ 2003]) with the products of genes involved in nuclear positioning ( p < 5.0 x 10-3).	gene_phenotype
70803	1	333897	5	NULL	NULL	NULL	NULL	YJL103c	NucleicAcid		is involved in		possibly			oxidative phosphorylation	Process				NULL		NULL	NULL	NULL	NULL	gw70_yeast_23_7_553_s_129	16710832	Only one unknown ORF was detected to be downregulated due to the  hap4 deletion (YJL103c); this already has a biological term annotation (oxidative phosphorylation)  which rests on indirect evidence.	gene_phenotype
70804	1	333898	5	NULL	NULL	0	NULL	YJL103c product	GP		is involved in		possibly			oxidative phosphorylation	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_7_553_s_262	16710832	The product of YJL103c was recently annotated to be involved in oxidative phosphorylation,  as inferred by sequence and structure similarity (Deng  et al., [ 2005]), and was defined as a zinc cluster protein by phenotype screening (Akache  et al., [ 2001]).	gene_phenotype
70805	2	333898	5	NULL	NULL	0	NULL	YJL103c product	GP		is a type of					zinc cluster protein	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_23_7_553_s_262	16710832	The product of YJL103c was recently annotated to be involved in oxidative phosphorylation,  as inferred by sequence and structure similarity (Deng  et al., [ 2005]), and was defined as a zinc cluster protein by phenotype screening (Akache  et al., [ 2001]).	gene_phenotype
70806	1	333901	5	NULL	NULL	NULL	NULL	Sen1p	GP	inactivation of	leads to					RNA	NucleicAcid	altered accumulation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6885_s_443	9819377	In addition, other RNAs have recently been shown to exhibit altered accumulation upon inactivation of Sen1p, including RNAs of unexpected size containing U5, snR40, and snR45 sequences ( 39).	gene_phenotype
70807	1	333903	5	NULL	NULL	0	NULL	YDR533Cp	NucleicAcid		is related to					Hsp31	GP	Escherichia coli			NULL		0	NULL	NULL	NULL	gw70_pnas_101_6_1531_s_6	14745011	The structure indicates that the closest relative to YDR533Cp is the  Escherichia coli heat shock protein Hsp31 (YedU), which has both chaperone and protease activity.	gene_phenotype
70808	2	333903	5	NULL	NULL	0	NULL	Hsp31	GP		is a type of					heat shock protein	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_6_1531_s_6	14745011	The structure indicates that the closest relative to YDR533Cp is the  Escherichia coli heat shock protein Hsp31 (YedU), which has both chaperone and protease activity.	gene_phenotype
70809	3	333903	5	NULL	NULL	0	NULL	YedU	GP		is a synonym of					Hsp31	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_6_1531_s_6	14745011	The structure indicates that the closest relative to YDR533Cp is the  Escherichia coli heat shock protein Hsp31 (YedU), which has both chaperone and protease activity.	gene_phenotype
70810	4	333903	5	NULL	NULL	0	NULL	Hsp31	GP		activates					chaperone	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_6_1531_s_6	14745011	The structure indicates that the closest relative to YDR533Cp is the  Escherichia coli heat shock protein Hsp31 (YedU), which has both chaperone and protease activity.	gene_phenotype
70811	5	333903	5	NULL	NULL	0	NULL	Hsp31	GP		activates					protease	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_6_1531_s_6	14745011	The structure indicates that the closest relative to YDR533Cp is the  Escherichia coli heat shock protein Hsp31 (YedU), which has both chaperone and protease activity.	gene_phenotype
70812	1	333908	5	NULL	NULL	NULL	NULL	YNR022c gene	GP		plays a role in					growth	Process				NULL		NULL	NULL	NULL	NULL	gw70_yeast_19_7_587_s_191	11967829	To our knowledge, this is the first report that  the  YNR022c and  YCR079w genes play some role in the growth at low and high temperatures, although the temperature-sensitive  growth of the  ptc1 disruptant has been reported previously (Maeda  et al., [ 1993]).	gene_phenotype
70813	2	333908	5	NULL	NULL	0	NULL	YCR079w gene	GP		plays a role in					growth	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_19_7_587_s_191	11967829	To our knowledge, this is the first report that  the  YNR022c and  YCR079w genes play some role in the growth at low and high temperatures, although the temperature-sensitive  growth of the  ptc1 disruptant has been reported previously (Maeda  et al., [ 1993]).	gene_phenotype
70814	1	333910	5	NULL	NULL	NULL	NULL	Yjl200c protein	GP		activates		probably			aconitate hydratase	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_3_762_s_203	16428434	For the protein Yjl200c, an uncharacterized open reading frame with postulated aconitate hydratase activity, an involvement in TCA cycle reactions seems plausible.	gene_phenotype
70815	2	333910	5	NULL	NULL	0	NULL	Yjl200c protein	GP		is involved in		probably			TCA cycle reactions	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_3_762_s_203	16428434	For the protein Yjl200c, an uncharacterized open reading frame with postulated aconitate hydratase activity, an involvement in TCA cycle reactions seems plausible.	gene_phenotype
70816	1	333911	5	NULL	NULL	0	NULL	YJL200c 	NucleicAcid		activates		possibly			aconitate hydratase	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_23_7_553_s_272	16710832	YJL200c was annotated with the term  aconitate hydratase activity  by sequence homology (Tatusov  et al., [ 2000]) and the location of its protein in the mitochondrion has been determined by direct  assay	gene_phenotype
70817	2	333911	5	NULL	NULL	0	NULL	Yjl200c protein	GP		is located in					mitochondria	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_23_7_553_s_272	16710832	YJL200c was annotated with the term  aconitate hydratase activity  by sequence homology (Tatusov  et al., [ 2000]) and the location of its protein in the mitochondrion has been determined by direct  assay	gene_phenotype
70818	1	333912	5	NULL	NULL	0	NULL	YGR284c	NucleicAcid		is the locus name of					ERV29	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_246	15334557	ERV29   YGR284c ER-Golgi transport vesicle protein	gene_phenotype
70819	2	333912	5	NULL	NULL	0	NULL	ERV29	GP		is a type of					ER-Golgi transport vesicle protein	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_21_11_927_s_246	15334557	ERV29   YGR284c ER-Golgi transport vesicle protein	gene_phenotype
70820	1	333915	5	NULL	NULL	0	NULL	YLR151c protein	GP		is a homolog of		functional			MutT	GP	S.cerevisiae			NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_32_18_5339_s_136	15475388	Purification of recombinant YLR151c protein and pyrophosphatase activity for the oxidized  deoxyribonucleotide triphosphates   Our observations from genetic approach strongly suggest that YLR151c is one of the important candidates for a functional homologue of MutT in  S.cerevisiae.	gene_phenotype
70821	1	333923	5	NULL	NULL	0	NULL	YLR151c	NucleicAcid		activates					pyrophosphatase	GP				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_32_18_5339_s_179	15475388	Effects of pH (left) and salt concentration (right) in the reaction mixture on pyrophosphatase  activity of YLR151c against 8-oxo-dGTP: 20 muM 8-oxo-dGTP was treated with 75 nM  GST-YLR151c fusion protein at 30 degrees C for 60 min at various pH and various salt  concentrations.	gene_phenotype
70822	1	333924	5	NULL	NULL	NULL	NULL	PCD1	GP	S. cerevisiae	is a type of					nudix hydrolase gene	GP	S. cerevisiae			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_42_32925_s_17	10922370	Here we show that the fifth  S. cerevisiae nudix hydrolase gene,  PCD1 (ORF YLR151C) on chromosome XII, encodes a protein with an entirely new enzyme activity: a  peroxisomal  coenzyme A  diphosphatase, Pcd1p, that cleaves 3''-phosphoadenosine 5''-monophosphate (3'',5''-ADP) from coenzyme A and CoA derivatives.	gene_phenotype
70823	2	333924	5	NULL	NULL	NULL	NULL	YLR151C	NucleicAcid	S. cerevisiae	is a type of					ORF	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_42_32925_s_17	10922370	Here we show that the fifth  S. cerevisiae nudix hydrolase gene,  PCD1 (ORF YLR151C) on chromosome XII, encodes a protein with an entirely new enzyme activity: a  peroxisomal  coenzyme A  diphosphatase, Pcd1p, that cleaves 3''-phosphoadenosine 5''-monophosphate (3'',5''-ADP) from coenzyme A and CoA derivatives.	gene_phenotype
70824	3	333924	5	NULL	NULL	NULL	NULL	YLR151C	NucleicAcid	S. cerevisiae	is the locus name of					PCD1	GP	S.cerevisiae			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_42_32925_s_17	10922370	Here we show that the fifth  S. cerevisiae nudix hydrolase gene,  PCD1 (ORF YLR151C) on chromosome XII, encodes a protein with an entirely new enzyme activity: a  peroxisomal  coenzyme A  diphosphatase, Pcd1p, that cleaves 3''-phosphoadenosine 5''-monophosphate (3'',5''-ADP) from coenzyme A and CoA derivatives.	gene_phenotype
70825	4	333924	5	NULL	NULL	NULL	NULL	YLR151C	NucleicAcid	S. cerevisiae	is located in					chromosome XII	Chromosome	S.cerevisiae			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_42_32925_s_17	10922370	Here we show that the fifth  S. cerevisiae nudix hydrolase gene,  PCD1 (ORF YLR151C) on chromosome XII, encodes a protein with an entirely new enzyme activity: a  peroxisomal  coenzyme A  diphosphatase, Pcd1p, that cleaves 3''-phosphoadenosine 5''-monophosphate (3'',5''-ADP) from coenzyme A and CoA derivatives.	gene_phenotype
70826	5	333924	5	NULL	NULL	NULL	NULL	YLR151C	NucleicAcid	S. cerevisiae	encodes for					peroxisomal coenzyme A diphosphatase	GP	S.cerevisiae			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_42_32925_s_17	10922370	Here we show that the fifth  S. cerevisiae nudix hydrolase gene,  PCD1 (ORF YLR151C) on chromosome XII, encodes a protein with an entirely new enzyme activity: a  peroxisomal  coenzyme A  diphosphatase, Pcd1p, that cleaves 3''-phosphoadenosine 5''-monophosphate (3'',5''-ADP) from coenzyme A and CoA derivatives.	gene_phenotype
70827	6	333924	5	NULL	NULL	0	NULL	peroxisomal coenzyme A diphosphatase	GP	S. cerevisiae	is a synonym of					Pcd1p	GP	S.cerevisiae			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_42_32925_s_17	10922370	Here we show that the fifth  S. cerevisiae nudix hydrolase gene,  PCD1 (ORF YLR151C) on chromosome XII, encodes a protein with an entirely new enzyme activity: a  peroxisomal  coenzyme A  diphosphatase, Pcd1p, that cleaves 3''-phosphoadenosine 5''-monophosphate (3'',5''-ADP) from coenzyme A and CoA derivatives.	gene_phenotype
70828	7	333924	5	NULL	NULL	0	NULL	3'',5''-ADP	Chemical		is					3''-phosphoadenosine 5''-monophosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_42_32925_s_17	10922370	Here we show that the fifth  S. cerevisiae nudix hydrolase gene,  PCD1 (ORF YLR151C) on chromosome XII, encodes a protein with an entirely new enzyme activity: a  peroxisomal  coenzyme A  diphosphatase, Pcd1p, that cleaves 3''-phosphoadenosine 5''-monophosphate (3'',5''-ADP) from coenzyme A and CoA derivatives.	gene_phenotype
70829	8	333924	5	NULL	NULL	0	NULL	3'',5''-ADP	Chemical		is cleaved from					coenzyme A 	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_42_32925_s_17	10922370	Here we show that the fifth  S. cerevisiae nudix hydrolase gene,  PCD1 (ORF YLR151C) on chromosome XII, encodes a protein with an entirely new enzyme activity: a  peroxisomal  coenzyme A  diphosphatase, Pcd1p, that cleaves 3''-phosphoadenosine 5''-monophosphate (3'',5''-ADP) from coenzyme A and CoA derivatives.	gene_phenotype
70830	9	333924	5	NULL	NULL	0	NULL	3'',5''-ADP	Chemical		is cleaved from					CoA derivatives	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_42_32925_s_17	10922370	Here we show that the fifth  S. cerevisiae nudix hydrolase gene,  PCD1 (ORF YLR151C) on chromosome XII, encodes a protein with an entirely new enzyme activity: a  peroxisomal  coenzyme A  diphosphatase, Pcd1p, that cleaves 3''-phosphoadenosine 5''-monophosphate (3'',5''-ADP) from coenzyme A and CoA derivatives.	gene_phenotype
70831	10	333924	5	NULL	NULL	NULL	NULL	Pcd1p	GP	S. cerevisiae	catalyzes					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_42_32925_s_17	10922370	Here we show that the fifth  S. cerevisiae nudix hydrolase gene,  PCD1 (ORF YLR151C) on chromosome XII, encodes a protein with an entirely new enzyme activity: a  peroxisomal  coenzyme A  diphosphatase, Pcd1p, that cleaves 3''-phosphoadenosine 5''-monophosphate (3'',5''-ADP) from coenzyme A and CoA derivatives.	gene_phenotype
70832	11	333924	5	NULL	NULL	0	NULL	Pcd1p	GP	S. cerevisiae	catalyzes					statement 9	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_42_32925_s_17	10922370	Here we show that the fifth  S. cerevisiae nudix hydrolase gene,  PCD1 (ORF YLR151C) on chromosome XII, encodes a protein with an entirely new enzyme activity: a  peroxisomal  coenzyme A  diphosphatase, Pcd1p, that cleaves 3''-phosphoadenosine 5''-monophosphate (3'',5''-ADP) from coenzyme A and CoA derivatives.	gene_phenotype
70833	1	333925	5	NULL	NULL	0	NULL	pheromone	GP	treatment of wt cells	increases					PGU1	GP	expression of			NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_115	10657304	PGU1 and  YLR042c also showed increased expression after pheromone treatment of wt cells ( Fig. 2B), which suggests overlap between the mating and filamentation responses.	gene_phenotype
70834	2	333925	5	NULL	NULL	0	NULL	pheromone	GP	treatment of wt cells	increases					YLR042c	NucleicAcid	expression of			NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_115	10657304	PGU1 and  YLR042c also showed increased expression after pheromone treatment of wt cells ( Fig. 2B), which suggests overlap between the mating and filamentation responses.	gene_phenotype
70835	3	333925	5	NULL	NULL	0	NULL	mating response	Process		overlaps with					filamentation response	Process				NULL		0	NULL	NULL	NULL	gw60_science_287_5454_873_s_115	10657304	PGU1 and  YLR042c also showed increased expression after pheromone treatment of wt cells ( Fig. 2B), which suggests overlap between the mating and filamentation responses.	gene_phenotype
70836	1	333927	5	NULL	NULL	0	NULL	FLO11	GP		doet not corelate with					invasive growth 	Process				NULL		0	NULL	NULL	NULL	gw70_genetics_165_3_997_s_301	14668360	For example, a genome-wide analysis of  TEC1-regulated genes in haploids  vs. diploids revealed just two common genes,  FLO11 and  YLR042C, both of which fail to correlate with invasive growth in other circumstances ( MADHANI et al. 1999  ;   PALECEK  et al. 2000  ).	gene_phenotype
70837	2	333927	5	NULL	NULL	0	NULL	YLR042C	NucleicAcid		doet not corelate with					invasive growth	Process				NULL		0	NULL	NULL	NULL	gw70_genetics_165_3_997_s_301	14668360	For example, a genome-wide analysis of  TEC1-regulated genes in haploids  vs. diploids revealed just two common genes,  FLO11 and  YLR042C, both of which fail to correlate with invasive growth in other circumstances ( MADHANI et al. 1999  ;   PALECEK  et al. 2000  ).	gene_phenotype
70838	1	333930	5	NULL	NULL	0	NULL	Campylobacter	Organism		infects					human	Organism				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_19_20327_s_10	14985343	Campylobacter infection in humans occurs primarily through the consumption of contaminated poultry products ( ).	gene_phenotype
70839	2	333930	5	NULL	NULL	0	NULL	statement 1	Process		through		primarily			poultry products	OrganismPart	consumption of;;contaminated			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_19_20327_s_10	14985343	Campylobacter infection in humans occurs primarily through the consumption of contaminated poultry products ( ).	gene_phenotype
70840	1	333932	5	NULL	NULL	0	NULL	YLL031c	NucleicAcid	depletion of	accumulates					GPI proteins	GP	immature 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24458_s_108	10823837	Depletion of YLL031c Leads to the Accumulation of Immature GPI Proteins-- If Gas1p does not receive a GPI anchor in the ER, it fails to be transported to the Golgi ( 25), because, as shown by  in vitro experiments using a vesicle budding assay, nonanchored Gas1p is not packaged into COPII-coated transport vesicles budding off the ER ( 26).	gene_phenotype
70841	2	333932	5	NULL	NULL	NULL	NULL	transport vesicles	CellComponent	COPII-coated	buds off from					ER	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24458_s_108	10823837	Depletion of YLL031c Leads to the Accumulation of Immature GPI Proteins-- If Gas1p does not receive a GPI anchor in the ER, it fails to be transported to the Golgi ( 25), because, as shown by  in vitro experiments using a vesicle budding assay, nonanchored Gas1p is not packaged into COPII-coated transport vesicles budding off the ER ( 26).	gene_phenotype
70842	3	333932	5	NULL	NULL	0	NULL	Gas1p	GP	nonanchored	is not packaged into					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24458_s_108	10823837	Depletion of YLL031c Leads to the Accumulation of Immature GPI Proteins-- If Gas1p does not receive a GPI anchor in the ER, it fails to be transported to the Golgi ( 25), because, as shown by  in vitro experiments using a vesicle budding assay, nonanchored Gas1p is not packaged into COPII-coated transport vesicles budding off the ER ( 26).	gene_phenotype
70855	4	333932	5	NULL	NULL	NULL	NULL	Gas1p	GP		is not transported to					Golgi	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_32_24458_s_108	10823837	Depletion of YLL031c Leads to the Accumulation of Immature GPI Proteins-- If Gas1p does not receive a GPI anchor in the ER, it fails to be transported to the Golgi ( 25), because, as shown by  in vitro experiments using a vesicle budding assay, nonanchored Gas1p is not packaged into COPII-coated transport vesicles budding off the ER ( 26).	gene_phenotype
70856	5	333932	5	NULL	NULL	0	NULL	Gas1p	GP		does not receive					GPI anchor	GP				NULL	ER	0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24458_s_108	10823837	Depletion of YLL031c Leads to the Accumulation of Immature GPI Proteins-- If Gas1p does not receive a GPI anchor in the ER, it fails to be transported to the Golgi ( 25), because, as shown by  in vitro experiments using a vesicle budding assay, nonanchored Gas1p is not packaged into COPII-coated transport vesicles budding off the ER ( 26).	gene_phenotype
70857	6	333932	5	NULL	NULL	0	NULL	statement 5	Process		leads to					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_32_24458_s_108	10823837	Depletion of YLL031c Leads to the Accumulation of Immature GPI Proteins-- If Gas1p does not receive a GPI anchor in the ER, it fails to be transported to the Golgi ( 25), because, as shown by  in vitro experiments using a vesicle budding assay, nonanchored Gas1p is not packaged into COPII-coated transport vesicles budding off the ER ( 26).	gene_phenotype
70858	1	333933	5	NULL	NULL	0	NULL	YAR031W	NucleicAcid	lack of	is not a consequence of					truncation	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_2_171_s_158	12518320	We concluded that the lack of YAR031W and of the rest of telomere-proximal ORFs  was not a consequence of a truncation, but rather of a recombination event that did  not implicate a gross change on the total length of the chromosome I left arm.	gene_phenotype
70859	2	333933	5	NULL	NULL	0	NULL	YAR031W	NucleicAcid	lack of	is consequence of					recombination event	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_2_171_s_158	12518320	We concluded that the lack of YAR031W and of the rest of telomere-proximal ORFs  was not a consequence of a truncation, but rather of a recombination event that did  not implicate a gross change on the total length of the chromosome I left arm.	gene_phenotype
70860	3	333933	5	NULL	NULL	0	NULL	statement 2	Process		does not change					chromosome I	Chromosome	total length of;;left arm of			NULL		0	NULL	NULL	NULL	gw70_yeast_20_2_171_s_158	12518320	We concluded that the lack of YAR031W and of the rest of telomere-proximal ORFs  was not a consequence of a truncation, but rather of a recombination event that did  not implicate a gross change on the total length of the chromosome I left arm.	gene_phenotype
70861	1	333934	5	NULL	NULL	0	NULL	Blm1	GP		is a synonym of					Bloom's Syndrome helicase	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_4_1724_s_377	14742710	Blm1 is the Bloom's Syndrome helicase homologous to budding yeast Sgs1, a ctf4delta interacting gene that also contributes to cohesion.	gene_phenotype
70862	2	333934	5	NULL	NULL	0	NULL	Bloom's Syndrome helicase	Process		is homologous to					Sgs1	GP	budding yeast			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_4_1724_s_377	14742710	Blm1 is the Bloom's Syndrome helicase homologous to budding yeast Sgs1, a ctf4delta interacting gene that also contributes to cohesion.	gene_phenotype
70863	3	333934	5	NULL	NULL	0	NULL	Sgs1	GP	budding yeast	interacts with					ctf4delta gene	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_4_1724_s_377	14742710	Blm1 is the Bloom's Syndrome helicase homologous to budding yeast Sgs1, a ctf4delta interacting gene that also contributes to cohesion.	gene_phenotype
70864	4	333934	5	NULL	NULL	0	NULL	ctf4delta gene	GP		contribute to					cohesion	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_4_1724_s_377	14742710	Blm1 is the Bloom's Syndrome helicase homologous to budding yeast Sgs1, a ctf4delta interacting gene that also contributes to cohesion.	gene_phenotype
70865	1	333935	5	NULL	NULL	0	NULL	Blm3p	GP		is a homolog of					PA200	GP				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_methods-enzymol_398_1_16275339_s_3	16275339	Homologs of PA200  have been found in rat, frog, birds, worms, and budding yeast, where it  is called Blm3p (now known as Blm10p), but not in Drosophila or fission  yeast.	gene_phenotype
70866	2	333935	5	NULL	NULL	0	NULL	Blm3p	GP		is a synonym of					Blm10p	GP				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_methods-enzymol_398_1_16275339_s_3	16275339	Homologs of PA200  have been found in rat, frog, birds, worms, and budding yeast, where it  is called Blm3p (now known as Blm10p), but not in Drosophila or fission  yeast.	gene_phenotype
70867	3	333935	5	NULL	NULL	0	NULL	Blm10p	GP		is present in					rat	Organism				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_methods-enzymol_398_1_16275339_s_3	16275339	Homologs of PA200  have been found in rat, frog, birds, worms, and budding yeast, where it  is called Blm3p (now known as Blm10p), but not in Drosophila or fission  yeast.	gene_phenotype
70868	4	333935	5	NULL	NULL	0	NULL	Blm10p	GP		is present in					frog	Organism				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_methods-enzymol_398_1_16275339_s_3	16275339	Homologs of PA200  have been found in rat, frog, birds, worms, and budding yeast, where it  is called Blm3p (now known as Blm10p), but not in Drosophila or fission  yeast.	gene_phenotype
70869	5	333935	5	NULL	NULL	0	NULL	Blm10p	GP		is present in					birds	Organism				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_methods-enzymol_398_1_16275339_s_3	16275339	Homologs of PA200  have been found in rat, frog, birds, worms, and budding yeast, where it  is called Blm3p (now known as Blm10p), but not in Drosophila or fission  yeast.	gene_phenotype
70870	6	333935	5	NULL	NULL	0	NULL	Blm10p	GP		is present in					worms	Organism				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_methods-enzymol_398_1_16275339_s_3	16275339	Homologs of PA200  have been found in rat, frog, birds, worms, and budding yeast, where it  is called Blm3p (now known as Blm10p), but not in Drosophila or fission  yeast.	gene_phenotype
70871	7	333935	5	NULL	NULL	0	NULL	Blm10p	GP		is present in					budding yeast	Organism				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_methods-enzymol_398_1_16275339_s_3	16275339	Homologs of PA200  have been found in rat, frog, birds, worms, and budding yeast, where it  is called Blm3p (now known as Blm10p), but not in Drosophila or fission  yeast.	gene_phenotype
70872	8	333935	5	NULL	NULL	0	NULL	Blm10p	GP		is not present in					Drosophila	Organism				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_methods-enzymol_398_1_16275339_s_3	16275339	Homologs of PA200  have been found in rat, frog, birds, worms, and budding yeast, where it  is called Blm3p (now known as Blm10p), but not in Drosophila or fission  yeast.	gene_phenotype
70873	9	333935	5	NULL	NULL	0	NULL	Blm10p	GP		is not present in					fission yeast	Organism				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_methods-enzymol_398_1_16275339_s_3	16275339	Homologs of PA200  have been found in rat, frog, birds, worms, and budding yeast, where it  is called Blm3p (now known as Blm10p), but not in Drosophila or fission  yeast.	gene_phenotype
70874	1	333936	5	NULL	NULL	0	NULL	YNR007c	NucleicAcid		is the locus name of					AUT1	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_79_s_288	12489128	YNR007c ( AUT1) is essential for autophagocytosis or transport of proteins from cytoplasm to vacuole  (Schlumpberger  et al., [ 1997]).	gene_phenotype
70875	2	333936	5	NULL	NULL	0	NULL	AUT1	GP		is essential for					autophagocytosis	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_79_s_288	12489128	YNR007c ( AUT1) is essential for autophagocytosis or transport of proteins from cytoplasm to vacuole  (Schlumpberger  et al., [ 1997]).	gene_phenotype
70876	3	333936	5	NULL	NULL	0	NULL	protein	GP		is transported from					cytoplasm	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_79_s_288	12489128	YNR007c ( AUT1) is essential for autophagocytosis or transport of proteins from cytoplasm to vacuole  (Schlumpberger  et al., [ 1997]).	gene_phenotype
70877	4	333936	5	NULL	NULL	0	NULL	protein	GP		is transported to					vacuole	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_79_s_288	12489128	YNR007c ( AUT1) is essential for autophagocytosis or transport of proteins from cytoplasm to vacuole  (Schlumpberger  et al., [ 1997]).	gene_phenotype
70878	5	333936	5	NULL	NULL	0	NULL	statement 3	Process		occurs along with					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_79_s_288	12489128	YNR007c ( AUT1) is essential for autophagocytosis or transport of proteins from cytoplasm to vacuole  (Schlumpberger  et al., [ 1997]).	gene_phenotype
70879	6	333936	5	NULL	NULL	0	NULL	AUT1	GP		is essential for					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_79_s_288	12489128	YNR007c ( AUT1) is essential for autophagocytosis or transport of proteins from cytoplasm to vacuole  (Schlumpberger  et al., [ 1997]).	gene_phenotype
70880	7	333936	5	NULL	NULL	0	NULL	AUT1	GP		is essential for					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_79_s_288	12489128	YNR007c ( AUT1) is essential for autophagocytosis or transport of proteins from cytoplasm to vacuole  (Schlumpberger  et al., [ 1997]).	gene_phenotype
70881	1	333942	5	NULL	NULL	0	NULL	piD261	GP	Saccharomyces cerevisiae	activates					Ser/Thr-specific protein kinase 	GP				NULL		0	NULL	NULL	NULL	gw60_genomeres_8_10_1038_s_33	9799791	This hypothesis is supported by biochemical data in the case of  Saccharomyces cerevisiae piD261 (YGR262C), which is a member of one of the identified protein families (see below) and has been shown to possess Ser/Thr-specific protein kinase activity (Stocchetto et al. 1997  ).	gene_phenotype
70882	2	333942	5	NULL	NULL	0	NULL	YGR262C	NucleicAcid	Saccharomyces cerevisiae	is the locus name of					piD261	GP	Saccharomyces cerevisiae			NULL		0	NULL	NULL	NULL	gw60_genomeres_8_10_1038_s_33	9799791	This hypothesis is supported by biochemical data in the case of  Saccharomyces cerevisiae piD261 (YGR262C), which is a member of one of the identified protein families (see below) and has been shown to possess Ser/Thr-specific protein kinase activity (Stocchetto et al. 1997  ).	gene_phenotype
70883	1	333943	5	NULL	NULL	0	NULL	YGR262C	NucleicAcid	Saccharomyces cerevisiae	is the locus name of					piD261 protein	GP	Saccharomyces cerevisiae			NULL		0	NULL	NULL	NULL	gw60_genomeres_8_10_1038_s_71	9799791	However, in light of the fact that the  S. cerevisiae piD261 (YGR262C) protein (which does not contain the APE motif) has been shown to possess Ser/Thr-specific protein kinase activity (Stocchetto et al. 1997  ), this element is apparently not strictly essential for protein kinase catalytic activity.	gene_phenotype
70884	2	333943	5	NULL	NULL	0	NULL	piD261 protein	GP	Saccharomyces cerevisiae	does not contain					APE motif	AminoAcid				NULL		0	NULL	NULL	NULL	gw60_genomeres_8_10_1038_s_71	9799791	However, in light of the fact that the  S. cerevisiae piD261 (YGR262C) protein (which does not contain the APE motif) has been shown to possess Ser/Thr-specific protein kinase activity (Stocchetto et al. 1997  ), this element is apparently not strictly essential for protein kinase catalytic activity.	gene_phenotype
70885	3	333943	5	NULL	NULL	0	NULL	piD261 protein	GP	Saccharomyces cerevisiae	activates					Ser/Thr-specific protein kinase	GP				NULL		0	NULL	NULL	NULL	gw60_genomeres_8_10_1038_s_71	9799791	However, in light of the fact that the  S. cerevisiae piD261 (YGR262C) protein (which does not contain the APE motif) has been shown to possess Ser/Thr-specific protein kinase activity (Stocchetto et al. 1997  ), this element is apparently not strictly essential for protein kinase catalytic activity.	gene_phenotype
70886	1	333948	5	NULL	NULL	0	NULL	ybr078w/ ecm33 cells	Cell	growth of	is sensitive to					temperature	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiollett_218_1_175_s_63	12583915	Temperature-sensitive growth of  ybr078w/ ecm33  cells	gene_phenotype
70887	1	333949	5	NULL	NULL	0	NULL	YBR078W	NucleicAcid		is the locus name of					ECM33	GP				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiollett_218_1_175_s_20	12583915	A disruptant strain of  YBR078W/ ECM33 exhibited a temperature-sensitive (ts) growth phenotype [  13] and the hypersensitivity to oxidative stress [  14].	gene_phenotype
70888	2	333949	5	NULL	NULL	0	NULL	ECM33	GP	growth of;;disruptant strain of	is sensitive to					temperature	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiollett_218_1_175_s_20	12583915	A disruptant strain of  YBR078W/ ECM33 exhibited a temperature-sensitive (ts) growth phenotype [  13] and the hypersensitivity to oxidative stress [  14].	gene_phenotype
70889	3	333949	5	NULL	NULL	0	NULL	ECM33	GP	growth of;;disruptant strain of	is hypersensitive to					oxidative stress	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiollett_218_1_175_s_20	12583915	A disruptant strain of  YBR078W/ ECM33 exhibited a temperature-sensitive (ts) growth phenotype [  13] and the hypersensitivity to oxidative stress [  14].	gene_phenotype
70890	1	333950	5	NULL	NULL	0	NULL	YBR078W	NucleicAcid		is the locus name of					ECM33	GP				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiollett_218_1_175_s_64	12583915	A deleted strain of  YBR078W/ ECM33 has shown a temperature-sensitive (ts) growth phenotype in a previous report [ 13].	gene_phenotype
70891	2	333950	5	NULL	NULL	0	NULL	ECM33 	GP	growth of;;deleted strain of	is sensitive to					temperature	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiollett_218_1_175_s_64	12583915	A deleted strain of  YBR078W/ ECM33 has shown a temperature-sensitive (ts) growth phenotype in a previous report [ 13].	gene_phenotype
70892	1	333952	5	NULL	NULL	0	NULL	YDL247w product	GP		is homologous to		highly			MAL61	GP				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_450_s_154	0009925567	The high levels of homology exhibited by the products of YDL247w and YJR160c to MAL61 and AGT1 suggest that these proteins play a role in alpha-glucoside transport.	gene_phenotype
70893	2	333952	5	NULL	NULL	0	NULL	YJR160c product	GP		is homologous to		highly			AGT1	GP				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_450_s_154	0009925567	The high levels of homology exhibited by the products of YDL247w and YJR160c to MAL61 and AGT1 suggest that these proteins play a role in alpha-glucoside transport.	gene_phenotype
70894	3	333952	5	NULL	NULL	0	NULL	YDL247w product	GP		plays a role in					alpha-glucoside	Chemical	transport of			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_450_s_154	0009925567	The high levels of homology exhibited by the products of YDL247w and YJR160c to MAL61 and AGT1 suggest that these proteins play a role in alpha-glucoside transport.	gene_phenotype
70895	4	333952	5	NULL	NULL	0	NULL	YJR160c product	GP		plays a role in					alpha-glucoside	Chemical	transport of			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_450_s_154	0009925567	The high levels of homology exhibited by the products of YDL247w and YJR160c to MAL61 and AGT1 suggest that these proteins play a role in alpha-glucoside transport.	gene_phenotype
70896	1	333953	5	NULL	NULL	0	NULL	YDL247w protein	GP		transports		low affinity;;possibly			maltose	Chemical				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_450_s_229	0009925567	One possible function of the proteins encoded by YDL247w and YJR160c might be in low-affinity transport of maltose, although this phenomenon has been ruled out in one study as an artifact ( 1).	gene_phenotype
70897	2	333953	5	NULL	NULL	0	NULL	YJR160c protein	GP		transports		low affinity;;possibly			maltose	Chemical				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_450_s_229	0009925567	One possible function of the proteins encoded by YDL247w and YJR160c might be in low-affinity transport of maltose, although this phenomenon has been ruled out in one study as an artifact ( 1).	gene_phenotype
70898	1	333954	5	NULL	NULL	0	NULL	YGL157W protein	GP		is similar to					oxidoreductases	GP				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_3_1_221_s_211	14871952	The protein encoded by  YGL157W is similar to oxidoreductases with dihydroflavanol 4-reductase activity (Gene Ontology Consortium, SGD;  http://www.geneontology.	gene_phenotype
70899	2	333954	5	NULL	NULL	0	NULL	YGL157W protein	GP		activates					dihydroflavanol 4-reductase	GP				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_3_1_221_s_211	14871952	The protein encoded by  YGL157W is similar to oxidoreductases with dihydroflavanol 4-reductase activity (Gene Ontology Consortium, SGD;  http://www.geneontology.	gene_phenotype
70900	1	333955	5	NULL	NULL	0	NULL	YdfG protein	GP	hypothetical;;E. coli	activates					serine dehydrogenase	GP				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1645_1_89_s_161	12535615	Two hypothetical proteins of  E. coli and  S. cerevisiae, YdfG and YMR226C, showed NADP+-dependent  -serine dehydrogenase activity.	gene_phenotype
70901	2	333955	5	NULL	NULL	0	NULL	statement 1	Process		is dependent on					NADP+	Chemical				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1645_1_89_s_161	12535615	Two hypothetical proteins of  E. coli and  S. cerevisiae, YdfG and YMR226C, showed NADP+-dependent  -serine dehydrogenase activity.	gene_phenotype
70902	3	333955	5	NULL	NULL	0	NULL	YMR226C protein	GP	hypothetical;;S. cerevisiae	activates					serine dehydrogenase	GP				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1645_1_89_s_161	12535615	Two hypothetical proteins of  E. coli and  S. cerevisiae, YdfG and YMR226C, showed NADP+-dependent  -serine dehydrogenase activity.	gene_phenotype
70903	4	333955	5	NULL	NULL	0	NULL	statement 3	Process		is dependent on					NADP+	Chemical				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1645_1_89_s_161	12535615	Two hypothetical proteins of  E. coli and  S. cerevisiae, YdfG and YMR226C, showed NADP+-dependent  -serine dehydrogenase activity.	gene_phenotype
70904	1	333958	5	NULL	NULL	0	NULL	RTM1	GP		mediates					TEV-specific resistance	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_97_1_489_s_215	10618445	Two hypotheses for how RTM1 mediates TEV-specific resistance are viable.	gene_phenotype
70905	1	333959	5	NULL	NULL	0	NULL	RTM1	GP		mediates					TEV	Organism	specific recognition of			NULL		0	NULL	NULL	NULL	gw60_pnas_96_2_772_s_221	9892709	The hypothesis that RTM1 and/or RTM2 mediate specific recognition of TEV and elicitation of silencing is worth testing.	gene_phenotype
70906	2	333959	5	NULL	NULL	0	NULL	RTM2	GP		mediates					TEV	Organism	specific recognition of			NULL		0	NULL	NULL	NULL	gw60_pnas_96_2_772_s_221	9892709	The hypothesis that RTM1 and/or RTM2 mediate specific recognition of TEV and elicitation of silencing is worth testing.	gene_phenotype
70907	1	333960	5	NULL	NULL	0	NULL	TEV	Organism		prevents					silencing signal	AminoAcid	systemic spread of;;sequence-specific			NULL		0	NULL	NULL	NULL	gw60_cell_103_1_157_s_262	11051555	Conceivably, the products of RTM1 and RTM2 could  affect the ability of TEV to prevent systemic spread of the sequence-specific  silencing signal (Chisholm et al., 2000   ).	gene_phenotype
70908	2	333960	5	NULL	NULL	0	NULL	RTM1	GP		affects					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_cell_103_1_157_s_262	11051555	Conceivably, the products of RTM1 and RTM2 could  affect the ability of TEV to prevent systemic spread of the sequence-specific  silencing signal (Chisholm et al., 2000   ).	gene_phenotype
70910	3	333960	5	NULL	NULL	0	NULL	RTM2 	GP		affects					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_cell_103_1_157_s_262	11051555	Conceivably, the products of RTM1 and RTM2 could  affect the ability of TEV to prevent systemic spread of the sequence-specific  silencing signal (Chisholm et al., 2000   ).	gene_phenotype
70911	1	333961	5	NULL	NULL	0	NULL	YFL007w	NucleicAcid	deletion of	does not affect					viability	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_19_8_699_s_79	12185839	Deletion of neither  YFL007w nor  YFL006w affects viability (Winzeler  et al., [ 1999]), indicating that thegene is not essential.	gene_phenotype
70912	2	333961	5	NULL	NULL	0	NULL	YFL006w	NucleicAcid	deletion of	does not affect					viability	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_19_8_699_s_79	12185839	Deletion of neither  YFL007w nor  YFL006w affects viability (Winzeler  et al., [ 1999]), indicating that thegene is not essential.	gene_phenotype
70913	1	333962	5	NULL	NULL	0	NULL	YFL007w protein	GP	purified	co-associates with					Sir4 protein	Process	purified			NULL		0	NULL	NULL	NULL	gw70_yeast_19_8_699_s_90	12185839	Systematic mass spectrometric analysis of purified protein  complexes have identified YFL007w and YFL006w in co-association with the chromatin  silencing regulator Sir4 (Ho  et al.  Nature 2002;  415: 180) and with the 26S proteasome subunit Scl1 (Gavin  et al.  Nature 2002;  415: 141).	gene_phenotype
70914	2	333962	5	NULL	NULL	0	NULL	YFL006w protein	GP	purified	co-associates with					Sir4 protein	GP	purified			NULL		0	NULL	NULL	NULL	gw70_yeast_19_8_699_s_90	12185839	Systematic mass spectrometric analysis of purified protein  complexes have identified YFL007w and YFL006w in co-association with the chromatin  silencing regulator Sir4 (Ho  et al.  Nature 2002;  415: 180) and with the 26S proteasome subunit Scl1 (Gavin  et al.  Nature 2002;  415: 141).	gene_phenotype
70915	3	333962	5	NULL	NULL	0	NULL	Sir4 	GP		is a type of					chromatin silencing regulator	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_19_8_699_s_90	12185839	Systematic mass spectrometric analysis of purified protein  complexes have identified YFL007w and YFL006w in co-association with the chromatin  silencing regulator Sir4 (Ho  et al.  Nature 2002;  415: 180) and with the 26S proteasome subunit Scl1 (Gavin  et al.  Nature 2002;  415: 141).	gene_phenotype
70916	4	333962	5	NULL	NULL	0	NULL	Scl1	GP		is a subunit of					26S proteasome	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_19_8_699_s_90	12185839	Systematic mass spectrometric analysis of purified protein  complexes have identified YFL007w and YFL006w in co-association with the chromatin  silencing regulator Sir4 (Ho  et al.  Nature 2002;  415: 180) and with the 26S proteasome subunit Scl1 (Gavin  et al.  Nature 2002;  415: 141).	gene_phenotype
70917	5	333962	5	NULL	NULL	0	NULL	YFL007w protein \t	GP	purified	co-associates with					Scl1 protein	GP	purified			NULL		0	NULL	NULL	NULL	gw70_yeast_19_8_699_s_90	12185839	Systematic mass spectrometric analysis of purified protein  complexes have identified YFL007w and YFL006w in co-association with the chromatin  silencing regulator Sir4 (Ho  et al.  Nature 2002;  415: 180) and with the 26S proteasome subunit Scl1 (Gavin  et al.  Nature 2002;  415: 141).	gene_phenotype
70918	6	333962	5	NULL	NULL	0	NULL	YFL006w protein	GP	purified	co-associates with					Scl1 protein	GP	purified			NULL		0	NULL	NULL	NULL	gw70_yeast_19_8_699_s_90	12185839	Systematic mass spectrometric analysis of purified protein  complexes have identified YFL007w and YFL006w in co-association with the chromatin  silencing regulator Sir4 (Ho  et al.  Nature 2002;  415: 180) and with the 26S proteasome subunit Scl1 (Gavin  et al.  Nature 2002;  415: 141).	gene_phenotype
70919	1	333964	5	NULL	NULL	0	NULL	snR85	NucleicAcid		is required for		potentially			psi modification	Process	guiding			NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_32_14_4281_s_225	15306656	Unfortunately, we were unable to determine whether the sixth verified RNA (snR85) is required for guiding its predicted psi modification.	gene_phenotype
71912	1	333965	5	NULL	NULL	0	NULL	184-nt 6 S	NucleicAcid	E. coli	modulates					promoter use	Process				NULL		0	NULL	NULL	NULL	gw60_science_296_5571_1260_s_21	12016301	[[ Process Example Function Reference     Transcription 184-nt  E. coli 6 S Modulates promoter use ]] ( 9,  14)   331-nt human 7SK  Inhibits transcription elongation factor P-TEFb ( 15,  16,  46)   875-nt human SRA Steroid receptor coactivator ( 12,  17)  Gene silencing  16,500-nt human  Xist Required for X-chromosome inactivation ( 12,  13)   ~100,000-nt human  Air Required for autosomal gene imprinting ( 11)  Replication 451-nt human telomerase RNA Core of telomerase and telomere template ( 18,  46)  RNA processing 377-nt  E. coli RNase P Catalytic core of RNase P ( 9,  19)   186-nt human U2 snRNA Core of spliceosome ( 20,  46)  RNA modification 102-nt  S. cerevisiae U18 C/D snoRNA Directs 2''- O-ribose methylation of target rRNA  ( 21,  47)   189-nt  S. cerevisiae snR8 H/ACA snoRNA Directs pseudouridylation of target rRNA ( 21,  47)   68-nt  T. brucei gCYb gRNA Directs the insertion and excision of uridines ( 23,  24,  48)  RNA stability 80-nt  E. coli RyhB sRNA Targets mRNAs for degradation?	gene_phenotype
71913	2	333965	5	NULL	NULL	0	NULL	331-nt 7SK	NucleicAcid	human	inhibits					P-TEFb	GP				NULL		0	NULL	NULL	NULL	gw60_science_296_5571_1260_s_21	12016301	[[ Process Example Function Reference     Transcription 184-nt  E. coli 6 S Modulates promoter use ]] ( 9,  14)   331-nt human 7SK  Inhibits transcription elongation factor P-TEFb ( 15,  16,  46)   875-nt human SRA Steroid receptor coactivator ( 12,  17)  Gene silencing  16,500-nt human  Xist Required for X-chromosome inactivation ( 12,  13)   ~100,000-nt human  Air Required for autosomal gene imprinting ( 11)  Replication 451-nt human telomerase RNA Core of telomerase and telomere template ( 18,  46)  RNA processing 377-nt  E. coli RNase P Catalytic core of RNase P ( 9,  19)   186-nt human U2 snRNA Core of spliceosome ( 20,  46)  RNA modification 102-nt  S. cerevisiae U18 C/D snoRNA Directs 2''- O-ribose methylation of target rRNA  ( 21,  47)   189-nt  S. cerevisiae snR8 H/ACA snoRNA Directs pseudouridylation of target rRNA ( 21,  47)   68-nt  T. brucei gCYb gRNA Directs the insertion and excision of uridines ( 23,  24,  48)  RNA stability 80-nt  E. coli RyhB sRNA Targets mRNAs for degradation?	gene_phenotype
71914	3	333965	5	NULL	NULL	0	NULL	P-TEFb	GP		is a type of					transcription elongation factor	GP				NULL		0	NULL	NULL	NULL	gw60_science_296_5571_1260_s_21	12016301	[[ Process Example Function Reference     Transcription 184-nt  E. coli 6 S Modulates promoter use ]] ( 9,  14)   331-nt human 7SK  Inhibits transcription elongation factor P-TEFb ( 15,  16,  46)   875-nt human SRA Steroid receptor coactivator ( 12,  17)  Gene silencing  16,500-nt human  Xist Required for X-chromosome inactivation ( 12,  13)   ~100,000-nt human  Air Required for autosomal gene imprinting ( 11)  Replication 451-nt human telomerase RNA Core of telomerase and telomere template ( 18,  46)  RNA processing 377-nt  E. coli RNase P Catalytic core of RNase P ( 9,  19)   186-nt human U2 snRNA Core of spliceosome ( 20,  46)  RNA modification 102-nt  S. cerevisiae U18 C/D snoRNA Directs 2''- O-ribose methylation of target rRNA  ( 21,  47)   189-nt  S. cerevisiae snR8 H/ACA snoRNA Directs pseudouridylation of target rRNA ( 21,  47)   68-nt  T. brucei gCYb gRNA Directs the insertion and excision of uridines ( 23,  24,  48)  RNA stability 80-nt  E. coli RyhB sRNA Targets mRNAs for degradation?	gene_phenotype
71915	4	333965	5	NULL	NULL	0	NULL	875-nt SRA	NucleicAcid	human	is a type of					Steroid receptor coactivator	GP				NULL		0	NULL	NULL	NULL	gw60_science_296_5571_1260_s_21	12016301	[[ Process Example Function Reference     Transcription 184-nt  E. coli 6 S Modulates promoter use ]] ( 9,  14)   331-nt human 7SK  Inhibits transcription elongation factor P-TEFb ( 15,  16,  46)   875-nt human SRA Steroid receptor coactivator ( 12,  17)  Gene silencing  16,500-nt human  Xist Required for X-chromosome inactivation ( 12,  13)   ~100,000-nt human  Air Required for autosomal gene imprinting ( 11)  Replication 451-nt human telomerase RNA Core of telomerase and telomere template ( 18,  46)  RNA processing 377-nt  E. coli RNase P Catalytic core of RNase P ( 9,  19)   186-nt human U2 snRNA Core of spliceosome ( 20,  46)  RNA modification 102-nt  S. cerevisiae U18 C/D snoRNA Directs 2''- O-ribose methylation of target rRNA  ( 21,  47)   189-nt  S. cerevisiae snR8 H/ACA snoRNA Directs pseudouridylation of target rRNA ( 21,  47)   68-nt  T. brucei gCYb gRNA Directs the insertion and excision of uridines ( 23,  24,  48)  RNA stability 80-nt  E. coli RyhB sRNA Targets mRNAs for degradation?	gene_phenotype
71916	5	333965	5	NULL	NULL	0	NULL	16,500-nt Xist	NucleicAcid	human	is required for					X-chromosome	Chromosome	inactivation of			NULL		0	NULL	NULL	NULL	gw60_science_296_5571_1260_s_21	12016301	[[ Process Example Function Reference     Transcription 184-nt  E. coli 6 S Modulates promoter use ]] ( 9,  14)   331-nt human 7SK  Inhibits transcription elongation factor P-TEFb ( 15,  16,  46)   875-nt human SRA Steroid receptor coactivator ( 12,  17)  Gene silencing  16,500-nt human  Xist Required for X-chromosome inactivation ( 12,  13)   ~100,000-nt human  Air Required for autosomal gene imprinting ( 11)  Replication 451-nt human telomerase RNA Core of telomerase and telomere template ( 18,  46)  RNA processing 377-nt  E. coli RNase P Catalytic core of RNase P ( 9,  19)   186-nt human U2 snRNA Core of spliceosome ( 20,  46)  RNA modification 102-nt  S. cerevisiae U18 C/D snoRNA Directs 2''- O-ribose methylation of target rRNA  ( 21,  47)   189-nt  S. cerevisiae snR8 H/ACA snoRNA Directs pseudouridylation of target rRNA ( 21,  47)   68-nt  T. brucei gCYb gRNA Directs the insertion and excision of uridines ( 23,  24,  48)  RNA stability 80-nt  E. coli RyhB sRNA Targets mRNAs for degradation?	gene_phenotype
71917	6	333965	5	NULL	NULL	0	NULL	100,000-nt Air	NucleicAcid	human	is required for					autosomal gene imprinting	Process				NULL		0	NULL	NULL	NULL	gw60_science_296_5571_1260_s_21	12016301	[[ Process Example Function Reference     Transcription 184-nt  E. coli 6 S Modulates promoter use ]] ( 9,  14)   331-nt human 7SK  Inhibits transcription elongation factor P-TEFb ( 15,  16,  46)   875-nt human SRA Steroid receptor coactivator ( 12,  17)  Gene silencing  16,500-nt human  Xist Required for X-chromosome inactivation ( 12,  13)   ~100,000-nt human  Air Required for autosomal gene imprinting ( 11)  Replication 451-nt human telomerase RNA Core of telomerase and telomere template ( 18,  46)  RNA processing 377-nt  E. coli RNase P Catalytic core of RNase P ( 9,  19)   186-nt human U2 snRNA Core of spliceosome ( 20,  46)  RNA modification 102-nt  S. cerevisiae U18 C/D snoRNA Directs 2''- O-ribose methylation of target rRNA  ( 21,  47)   189-nt  S. cerevisiae snR8 H/ACA snoRNA Directs pseudouridylation of target rRNA ( 21,  47)   68-nt  T. brucei gCYb gRNA Directs the insertion and excision of uridines ( 23,  24,  48)  RNA stability 80-nt  E. coli RyhB sRNA Targets mRNAs for degradation?	gene_phenotype
71918	7	333965	5	NULL	NULL	0	NULL	451-nt telomerase RNA	NucleicAcid	human	is the core of					telomerase	GP				NULL		0	NULL	NULL	NULL	gw60_science_296_5571_1260_s_21	12016301	[[ Process Example Function Reference     Transcription 184-nt  E. coli 6 S Modulates promoter use ]] ( 9,  14)   331-nt human 7SK  Inhibits transcription elongation factor P-TEFb ( 15,  16,  46)   875-nt human SRA Steroid receptor coactivator ( 12,  17)  Gene silencing  16,500-nt human  Xist Required for X-chromosome inactivation ( 12,  13)   ~100,000-nt human  Air Required for autosomal gene imprinting ( 11)  Replication 451-nt human telomerase RNA Core of telomerase and telomere template ( 18,  46)  RNA processing 377-nt  E. coli RNase P Catalytic core of RNase P ( 9,  19)   186-nt human U2 snRNA Core of spliceosome ( 20,  46)  RNA modification 102-nt  S. cerevisiae U18 C/D snoRNA Directs 2''- O-ribose methylation of target rRNA  ( 21,  47)   189-nt  S. cerevisiae snR8 H/ACA snoRNA Directs pseudouridylation of target rRNA ( 21,  47)   68-nt  T. brucei gCYb gRNA Directs the insertion and excision of uridines ( 23,  24,  48)  RNA stability 80-nt  E. coli RyhB sRNA Targets mRNAs for degradation?	gene_phenotype
71919	8	333965	5	NULL	NULL	0	NULL	451-nt telomerase RNA	NucleicAcid	human	is the core of					telomere template	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_science_296_5571_1260_s_21	12016301	[[ Process Example Function Reference     Transcription 184-nt  E. coli 6 S Modulates promoter use ]] ( 9,  14)   331-nt human 7SK  Inhibits transcription elongation factor P-TEFb ( 15,  16,  46)   875-nt human SRA Steroid receptor coactivator ( 12,  17)  Gene silencing  16,500-nt human  Xist Required for X-chromosome inactivation ( 12,  13)   ~100,000-nt human  Air Required for autosomal gene imprinting ( 11)  Replication 451-nt human telomerase RNA Core of telomerase and telomere template ( 18,  46)  RNA processing 377-nt  E. coli RNase P Catalytic core of RNase P ( 9,  19)   186-nt human U2 snRNA Core of spliceosome ( 20,  46)  RNA modification 102-nt  S. cerevisiae U18 C/D snoRNA Directs 2''- O-ribose methylation of target rRNA  ( 21,  47)   189-nt  S. cerevisiae snR8 H/ACA snoRNA Directs pseudouridylation of target rRNA ( 21,  47)   68-nt  T. brucei gCYb gRNA Directs the insertion and excision of uridines ( 23,  24,  48)  RNA stability 80-nt  E. coli RyhB sRNA Targets mRNAs for degradation?	gene_phenotype
71920	9	333965	5	NULL	NULL	0	NULL	377-nt RNase P	NucleicAcid	E. coli	is the catalytic core of					RNase P	GP				NULL		0	NULL	NULL	NULL	gw60_science_296_5571_1260_s_21	12016301	[[ Process Example Function Reference     Transcription 184-nt  E. coli 6 S Modulates promoter use ]] ( 9,  14)   331-nt human 7SK  Inhibits transcription elongation factor P-TEFb ( 15,  16,  46)   875-nt human SRA Steroid receptor coactivator ( 12,  17)  Gene silencing  16,500-nt human  Xist Required for X-chromosome inactivation ( 12,  13)   ~100,000-nt human  Air Required for autosomal gene imprinting ( 11)  Replication 451-nt human telomerase RNA Core of telomerase and telomere template ( 18,  46)  RNA processing 377-nt  E. coli RNase P Catalytic core of RNase P ( 9,  19)   186-nt human U2 snRNA Core of spliceosome ( 20,  46)  RNA modification 102-nt  S. cerevisiae U18 C/D snoRNA Directs 2''- O-ribose methylation of target rRNA  ( 21,  47)   189-nt  S. cerevisiae snR8 H/ACA snoRNA Directs pseudouridylation of target rRNA ( 21,  47)   68-nt  T. brucei gCYb gRNA Directs the insertion and excision of uridines ( 23,  24,  48)  RNA stability 80-nt  E. coli RyhB sRNA Targets mRNAs for degradation?	gene_phenotype
71921	10	333965	5	NULL	NULL	0	NULL	186-nt U2snRNA	NucleicAcid	human	is the core of					spliceosome	CellComponent				NULL		0	NULL	NULL	NULL	gw60_science_296_5571_1260_s_21	12016301	[[ Process Example Function Reference     Transcription 184-nt  E. coli 6 S Modulates promoter use ]] ( 9,  14)   331-nt human 7SK  Inhibits transcription elongation factor P-TEFb ( 15,  16,  46)   875-nt human SRA Steroid receptor coactivator ( 12,  17)  Gene silencing  16,500-nt human  Xist Required for X-chromosome inactivation ( 12,  13)   ~100,000-nt human  Air Required for autosomal gene imprinting ( 11)  Replication 451-nt human telomerase RNA Core of telomerase and telomere template ( 18,  46)  RNA processing 377-nt  E. coli RNase P Catalytic core of RNase P ( 9,  19)   186-nt human U2 snRNA Core of spliceosome ( 20,  46)  RNA modification 102-nt  S. cerevisiae U18 C/D snoRNA Directs 2''- O-ribose methylation of target rRNA  ( 21,  47)   189-nt  S. cerevisiae snR8 H/ACA snoRNA Directs pseudouridylation of target rRNA ( 21,  47)   68-nt  T. brucei gCYb gRNA Directs the insertion and excision of uridines ( 23,  24,  48)  RNA stability 80-nt  E. coli RyhB sRNA Targets mRNAs for degradation?	gene_phenotype
71922	11	333965	5	NULL	NULL	0	NULL	102-nt U18 C/D snoRNA	NucleicAcid	S. cerevisiae	directs					target rRNA	NucleicAcid	2''- O-ribose methylation of			NULL		0	NULL	NULL	NULL	gw60_science_296_5571_1260_s_21	12016301	[[ Process Example Function Reference     Transcription 184-nt  E. coli 6 S Modulates promoter use ]] ( 9,  14)   331-nt human 7SK  Inhibits transcription elongation factor P-TEFb ( 15,  16,  46)   875-nt human SRA Steroid receptor coactivator ( 12,  17)  Gene silencing  16,500-nt human  Xist Required for X-chromosome inactivation ( 12,  13)   ~100,000-nt human  Air Required for autosomal gene imprinting ( 11)  Replication 451-nt human telomerase RNA Core of telomerase and telomere template ( 18,  46)  RNA processing 377-nt  E. coli RNase P Catalytic core of RNase P ( 9,  19)   186-nt human U2 snRNA Core of spliceosome ( 20,  46)  RNA modification 102-nt  S. cerevisiae U18 C/D snoRNA Directs 2''- O-ribose methylation of target rRNA  ( 21,  47)   189-nt  S. cerevisiae snR8 H/ACA snoRNA Directs pseudouridylation of target rRNA ( 21,  47)   68-nt  T. brucei gCYb gRNA Directs the insertion and excision of uridines ( 23,  24,  48)  RNA stability 80-nt  E. coli RyhB sRNA Targets mRNAs for degradation?	gene_phenotype
71923	12	333965	5	NULL	NULL	0	NULL	189-nt snR8 H/ACA snoRNA	NucleicAcid	S. cerevisiae	directs					target rRNA	NucleicAcid	pseudouridylation of			NULL		0	NULL	NULL	NULL	gw60_science_296_5571_1260_s_21	12016301	[[ Process Example Function Reference     Transcription 184-nt  E. coli 6 S Modulates promoter use ]] ( 9,  14)   331-nt human 7SK  Inhibits transcription elongation factor P-TEFb ( 15,  16,  46)   875-nt human SRA Steroid receptor coactivator ( 12,  17)  Gene silencing  16,500-nt human  Xist Required for X-chromosome inactivation ( 12,  13)   ~100,000-nt human  Air Required for autosomal gene imprinting ( 11)  Replication 451-nt human telomerase RNA Core of telomerase and telomere template ( 18,  46)  RNA processing 377-nt  E. coli RNase P Catalytic core of RNase P ( 9,  19)   186-nt human U2 snRNA Core of spliceosome ( 20,  46)  RNA modification 102-nt  S. cerevisiae U18 C/D snoRNA Directs 2''- O-ribose methylation of target rRNA  ( 21,  47)   189-nt  S. cerevisiae snR8 H/ACA snoRNA Directs pseudouridylation of target rRNA ( 21,  47)   68-nt  T. brucei gCYb gRNA Directs the insertion and excision of uridines ( 23,  24,  48)  RNA stability 80-nt  E. coli RyhB sRNA Targets mRNAs for degradation?	gene_phenotype
71924	13	333965	5	NULL	NULL	0	NULL	68-nt gCYb gRNA	NucleicAcid	T. brucei	directs					uridine	NucleicAcid	insertion of;;excision of			NULL		0	NULL	NULL	NULL	gw60_science_296_5571_1260_s_21	12016301	[[ Process Example Function Reference     Transcription 184-nt  E. coli 6 S Modulates promoter use ]] ( 9,  14)   331-nt human 7SK  Inhibits transcription elongation factor P-TEFb ( 15,  16,  46)   875-nt human SRA Steroid receptor coactivator ( 12,  17)  Gene silencing  16,500-nt human  Xist Required for X-chromosome inactivation ( 12,  13)   ~100,000-nt human  Air Required for autosomal gene imprinting ( 11)  Replication 451-nt human telomerase RNA Core of telomerase and telomere template ( 18,  46)  RNA processing 377-nt  E. coli RNase P Catalytic core of RNase P ( 9,  19)   186-nt human U2 snRNA Core of spliceosome ( 20,  46)  RNA modification 102-nt  S. cerevisiae U18 C/D snoRNA Directs 2''- O-ribose methylation of target rRNA  ( 21,  47)   189-nt  S. cerevisiae snR8 H/ACA snoRNA Directs pseudouridylation of target rRNA ( 21,  47)   68-nt  T. brucei gCYb gRNA Directs the insertion and excision of uridines ( 23,  24,  48)  RNA stability 80-nt  E. coli RyhB sRNA Targets mRNAs for degradation?	gene_phenotype
71925	15	333965	5	NULL	NULL	0	NULL	80-nt RyhB sRNA	NucleicAcid	E. coli	is required for					statement 14	Process				NULL		0	NULL	NULL	NULL	gw60_science_296_5571_1260_s_21	12016301	[[ Process Example Function Reference     Transcription 184-nt  E. coli 6 S Modulates promoter use ]] ( 9,  14)   331-nt human 7SK  Inhibits transcription elongation factor P-TEFb ( 15,  16,  46)   875-nt human SRA Steroid receptor coactivator ( 12,  17)  Gene silencing  16,500-nt human  Xist Required for X-chromosome inactivation ( 12,  13)   ~100,000-nt human  Air Required for autosomal gene imprinting ( 11)  Replication 451-nt human telomerase RNA Core of telomerase and telomere template ( 18,  46)  RNA processing 377-nt  E. coli RNase P Catalytic core of RNase P ( 9,  19)   186-nt human U2 snRNA Core of spliceosome ( 20,  46)  RNA modification 102-nt  S. cerevisiae U18 C/D snoRNA Directs 2''- O-ribose methylation of target rRNA  ( 21,  47)   189-nt  S. cerevisiae snR8 H/ACA snoRNA Directs pseudouridylation of target rRNA ( 21,  47)   68-nt  T. brucei gCYb gRNA Directs the insertion and excision of uridines ( 23,  24,  48)  RNA stability 80-nt  E. coli RyhB sRNA Targets mRNAs for degradation?	gene_phenotype
71926	14	333965	5	NULL	NULL	0	NULL	mRNA	NucleicAcid		is targeted for					degradation	Process				NULL		0	NULL	NULL	NULL	gw60_science_296_5571_1260_s_21	12016301	[[ Process Example Function Reference     Transcription 184-nt  E. coli 6 S Modulates promoter use ]] ( 9,  14)   331-nt human 7SK  Inhibits transcription elongation factor P-TEFb ( 15,  16,  46)   875-nt human SRA Steroid receptor coactivator ( 12,  17)  Gene silencing  16,500-nt human  Xist Required for X-chromosome inactivation ( 12,  13)   ~100,000-nt human  Air Required for autosomal gene imprinting ( 11)  Replication 451-nt human telomerase RNA Core of telomerase and telomere template ( 18,  46)  RNA processing 377-nt  E. coli RNase P Catalytic core of RNase P ( 9,  19)   186-nt human U2 snRNA Core of spliceosome ( 20,  46)  RNA modification 102-nt  S. cerevisiae U18 C/D snoRNA Directs 2''- O-ribose methylation of target rRNA  ( 21,  47)   189-nt  S. cerevisiae snR8 H/ACA snoRNA Directs pseudouridylation of target rRNA ( 21,  47)   68-nt  T. brucei gCYb gRNA Directs the insertion and excision of uridines ( 23,  24,  48)  RNA stability 80-nt  E. coli RyhB sRNA Targets mRNAs for degradation?	gene_phenotype
70920	1	333966	5	NULL	NULL	0	NULL	YGR280c gene	GP		is essential for					yeast	Organism	vegetative growth of			NULL	rich medium	0	NULL	NULL	NULL	gw70_yeast_20_1_79_s_5	12489128	Tetrad analysis, following  sporulation of the heterozygous disruptants, revealed that YGR280c and YNL006w are  essential genes for vegetative yeast growth in rich medium.	gene_phenotype
70921	2	333966	5	NULL	NULL	0	NULL	YNL006w gene	GP		is essential for					yeast	Organism	vegetative growth of			NULL	rich medium	0	NULL	NULL	NULL	gw70_yeast_20_1_79_s_5	12489128	Tetrad analysis, following  sporulation of the heterozygous disruptants, revealed that YGR280c and YNL006w are  essential genes for vegetative yeast growth in rich medium.	gene_phenotype
70925	4	333969	5	NULL	NULL	0	NULL	YGR280c	NucleicAcid		is a type of					ORF	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_79_s_293	12489128	The conclusion of the present study is that two of the 12 ORFs analysed are essential  for yeast viability (YGR280c and YNL006w).	gene_phenotype
70927	3	333969	5	NULL	NULL	0	NULL	YGR280c	NucleicAcid		is a type of					ORF	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_79_s_293	12489128	The conclusion of the present study is that two of the 12 ORFs analysed are essential  for yeast viability (YGR280c and YNL006w).	gene_phenotype
70929	2	333969	5	NULL	NULL	NULL	NULL	YNL006w	NucleicAcid		is essential for					yeast	Organism	viability of			NULL		NULL	NULL	NULL	NULL	gw70_yeast_20_1_79_s_293	12489128	The conclusion of the present study is that two of the 12 ORFs analysed are essential  for yeast viability (YGR280c and YNL006w).	gene_phenotype
70930	1	333969	5	NULL	NULL	0	NULL	YGR280c	NucleicAcid		is essential for					yeast	Organism	viability of			NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_79_s_293	12489128	The conclusion of the present study is that two of the 12 ORFs analysed are essential  for yeast viability (YGR280c and YNL006w).	gene_phenotype
71040	1	333971	5	NULL	NULL	0	NULL	permeases	GP		is transported from					Golgi	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_79_s_7	12489128	The protein encoded by  YNL006w ( LST8) is now known to be involved in transport of permeases from the Golgi to the plasma  membrane.	gene_phenotype
71043	2	333971	5	NULL	NULL	0	NULL	permeases	GP		is transported to					plasma membrane	CellComponent				NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_79_s_7	12489128	The protein encoded by  YNL006w ( LST8) is now known to be involved in transport of permeases from the Golgi to the plasma  membrane.	gene_phenotype
71045	3	333971	5	NULL	NULL	0	NULL	statement 1	Process		occurs along with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_79_s_7	12489128	The protein encoded by  YNL006w ( LST8) is now known to be involved in transport of permeases from the Golgi to the plasma  membrane.	gene_phenotype
71047	4	333971	5	NULL	NULL	0	NULL	LST8 protein	GP		is encoded by					YNL006w	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_79_s_7	12489128	The protein encoded by  YNL006w ( LST8) is now known to be involved in transport of permeases from the Golgi to the plasma  membrane.	gene_phenotype
71048	5	333971	5	NULL	NULL	0	NULL	LST8 protein	GP		is involved in					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_79_s_7	12489128	The protein encoded by  YNL006w ( LST8) is now known to be involved in transport of permeases from the Golgi to the plasma  membrane.	gene_phenotype
71050	6	333971	5	NULL	NULL	0	NULL	LST8 protein	GP		is involved in					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_79_s_7	12489128	The protein encoded by  YNL006w ( LST8) is now known to be involved in transport of permeases from the Golgi to the plasma  membrane.	gene_phenotype
71052	1	333972	5	NULL	NULL	0	NULL	haploid YNL006w	NucleicAcid	disruptants 	is not impaired in					spore	Cell	germination of			NULL		0	NULL	NULL	NULL	gw70_yeast_20_1_79_s_248	12489128	Microscopic analysis revealed that haploid YNL006w disruptants were not impaired  in spore germination, but stopped growth after the formation of microcolonies.	gene_phenotype
71053	1	333975	5	NULL	NULL	0	NULL	cap structure	NucleicAcid		protects					RNA	NucleicAcid	5' end of			NULL		0	NULL	NULL	NULL	gw60_embo_18_2_457_s_78	9889201	Collectively, our results demonstrate that the cap structure, most likely by protecting the 5' end of the RNA, plays an important role in the accumulation of the wild-type snR5 and the mutant snR36- S1 and snR36- S2 box H/ACA snoRNAs.	gene_phenotype
71054	2	333975	5	NULL	NULL	0	NULL	cap structure	NucleicAcid		plays a role in		important			snR5	NucleicAcid	accumulation of;;wild-type			NULL		0	NULL	NULL	NULL	gw60_embo_18_2_457_s_78	9889201	Collectively, our results demonstrate that the cap structure, most likely by protecting the 5' end of the RNA, plays an important role in the accumulation of the wild-type snR5 and the mutant snR36- S1 and snR36- S2 box H/ACA snoRNAs.	gene_phenotype
71055	3	333975	5	NULL	NULL	NULL	NULL	statement 2	Process		via		most likely			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_2_457_s_78	9889201	Collectively, our results demonstrate that the cap structure, most likely by protecting the 5' end of the RNA, plays an important role in the accumulation of the wild-type snR5 and the mutant snR36- S1 and snR36- S2 box H/ACA snoRNAs.	gene_phenotype
71056	4	333975	5	NULL	NULL	0	NULL	cap structure	NucleicAcid		plays a role in		important			snR36- S1	NucleicAcid	accumulation of;;mutant			NULL		0	NULL	NULL	NULL	gw60_embo_18_2_457_s_78	9889201	Collectively, our results demonstrate that the cap structure, most likely by protecting the 5' end of the RNA, plays an important role in the accumulation of the wild-type snR5 and the mutant snR36- S1 and snR36- S2 box H/ACA snoRNAs.	gene_phenotype
71057	5	333975	5	NULL	NULL	0	NULL	statement 4	Process		via					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_2_457_s_78	9889201	Collectively, our results demonstrate that the cap structure, most likely by protecting the 5' end of the RNA, plays an important role in the accumulation of the wild-type snR5 and the mutant snR36- S1 and snR36- S2 box H/ACA snoRNAs.	gene_phenotype
71058	6	333975	5	NULL	NULL	0	NULL	cap structure	NucleicAcid		plays a role in		important			snR36- S2	NucleicAcid	accumulation of;;mutant		box H/ACA	NULL		0	NULL	NULL	NULL	gw60_embo_18_2_457_s_78	9889201	Collectively, our results demonstrate that the cap structure, most likely by protecting the 5' end of the RNA, plays an important role in the accumulation of the wild-type snR5 and the mutant snR36- S1 and snR36- S2 box H/ACA snoRNAs.	gene_phenotype
71059	7	333975	5	NULL	NULL	0	NULL	statement 6	Process		via					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_2_457_s_78	9889201	Collectively, our results demonstrate that the cap structure, most likely by protecting the 5' end of the RNA, plays an important role in the accumulation of the wild-type snR5 and the mutant snR36- S1 and snR36- S2 box H/ACA snoRNAs.	gene_phenotype
71060	8	333975	5	NULL	NULL	0	NULL	snR36- S2	NucleicAcid		is a type of					snoRNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_embo_18_2_457_s_78	9889201	Collectively, our results demonstrate that the cap structure, most likely by protecting the 5' end of the RNA, plays an important role in the accumulation of the wild-type snR5 and the mutant snR36- S1 and snR36- S2 box H/ACA snoRNAs.	gene_phenotype
71061	9	333975	5	NULL	NULL	0	NULL	snR36- S1	NucleicAcid		is a type of					snoRNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_embo_18_2_457_s_78	9889201	Collectively, our results demonstrate that the cap structure, most likely by protecting the 5' end of the RNA, plays an important role in the accumulation of the wild-type snR5 and the mutant snR36- S1 and snR36- S2 box H/ACA snoRNAs.	gene_phenotype
71062	1	333977	5	NULL	NULL	0	NULL	ycl012c ::G418	NucleicAcid	mutant	does not show					vegetative growth	Process	phenotypic change;;normal			NULL		0	NULL	NULL	NULL	gw70_yeast_20_8_731_s_209	12794934	The  ycl012c ::G418 mutant does not show any phenotypic change in normal vegetative growth, mating, or  sporulation.	gene_phenotype
71063	2	333977	5	NULL	NULL	0	NULL	ycl012c ::G418	NucleicAcid	mutant	does not show					mating	Process	phenotypic change;;normal			NULL		0	NULL	NULL	NULL	gw70_yeast_20_8_731_s_209	12794934	The  ycl012c ::G418 mutant does not show any phenotypic change in normal vegetative growth, mating, or  sporulation.	gene_phenotype
71064	3	333977	5	NULL	NULL	0	NULL	ycl012c ::G418	NucleicAcid	mutant	does not show					sporulation	Process	phenotypic change;;normal			NULL		0	NULL	NULL	NULL	gw70_yeast_20_8_731_s_209	12794934	The  ycl012c ::G418 mutant does not show any phenotypic change in normal vegetative growth, mating, or  sporulation.	gene_phenotype
71065	1	333979	5	NULL	NULL	0	NULL	silencing	Process		is mediated by					Sir protein	GP				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_32_17_5206_s_143	15459290	When tested alongside the  HMR-tRNA in the  MATa1 reporter gene assay,  TRT2 showed a partial barrier activity to Sir protein-mediated silencing ( ), while it appears to completely prevent the spread of alpha2 operator repression in this study.	gene_phenotype
71066	2	333979	5	NULL	NULL	0	NULL	partial barrier activity	Process		is shown to					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_32_17_5206_s_143	15459290	When tested alongside the  HMR-tRNA in the  MATa1 reporter gene assay,  TRT2 showed a partial barrier activity to Sir protein-mediated silencing ( ), while it appears to completely prevent the spread of alpha2 operator repression in this study.	gene_phenotype
71067	3	333979	5	NULL	NULL	0	NULL	TRT2	GP		plays a role in					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_32_17_5206_s_143	15459290	When tested alongside the  HMR-tRNA in the  MATa1 reporter gene assay,  TRT2 showed a partial barrier activity to Sir protein-mediated silencing ( ), while it appears to completely prevent the spread of alpha2 operator repression in this study.	gene_phenotype
71068	4	333979	5	NULL	NULL	0	NULL	TRT2	GP		prevents		completely			alpha2	GP	spread of;;repression of		operator	NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_32_17_5206_s_143	15459290	When tested alongside the  HMR-tRNA in the  MATa1 reporter gene assay,  TRT2 showed a partial barrier activity to Sir protein-mediated silencing ( ), while it appears to completely prevent the spread of alpha2 operator repression in this study.	gene_phenotype
71069	1	333980	5	NULL	NULL	0	NULL	MATa1	GP		is derepressed in					sir1	GP	mutant			NULL		0	NULL	NULL	NULL	gw60_molcell_6_4_769_s_54	11090616	[In new window] We also examined silencing of a  URA3 gene at  HMR by monitoring the growth of cells on medium lacking uracil or containing 5-FOA. As seen for  MATa1, the  URA3 gene at  HMR was derepressed in the  sir1 mutants (see   Figure 1).	gene_phenotype
71070	2	333980	5	NULL	NULL	0	NULL	URA3 gene	GP		is present in					HMR	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_molcell_6_4_769_s_54	11090616	[In new window] We also examined silencing of a  URA3 gene at  HMR by monitoring the growth of cells on medium lacking uracil or containing 5-FOA. As seen for  MATa1, the  URA3 gene at  HMR was derepressed in the  sir1 mutants (see   Figure 1).	gene_phenotype
71071	3	333980	5	NULL	NULL	0	NULL	URA3 gene	GP		is derepressed in					sir1	GP	mutant			NULL		0	NULL	NULL	NULL	gw60_molcell_6_4_769_s_54	11090616	[In new window] We also examined silencing of a  URA3 gene at  HMR by monitoring the growth of cells on medium lacking uracil or containing 5-FOA. As seen for  MATa1, the  URA3 gene at  HMR was derepressed in the  sir1 mutants (see   Figure 1).	gene_phenotype
71902	1	333982	5	NULL	NULL	0	NULL	HMR-tRNA	NucleicAcid		blocks					MATa1	GP	repression of			NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_32_17_5206_s_142	15459290	We have previously shown that the  HMR-tRNA ( tRNA Thr [AGU] CR1) acts as a barrier to the spread of silencing at the  HMR locus, as it blocks repression of a  MATa1 reporter gene when juxtaposed between the gene and the silencer, and its deletion from the natural chromosome leads to a 60% reduction of expression of the downstream  GIT1 gene ( ).	gene_phenotype
71903	2	333982	5	NULL	NULL	0	NULL	MATa1	GP		is a type of					repressor gene	GP				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_32_17_5206_s_142	15459290	We have previously shown that the  HMR-tRNA ( tRNA Thr [AGU] CR1) acts as a barrier to the spread of silencing at the  HMR locus, as it blocks repression of a  MATa1 reporter gene when juxtaposed between the gene and the silencer, and its deletion from the natural chromosome leads to a 60% reduction of expression of the downstream  GIT1 gene ( ).	gene_phenotype
71904	3	333982	5	NULL	NULL	0	NULL	HMR-tRNA	NucleicAcid		is juxtaposed between					gene	GP				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_32_17_5206_s_142	15459290	We have previously shown that the  HMR-tRNA ( tRNA Thr [AGU] CR1) acts as a barrier to the spread of silencing at the  HMR locus, as it blocks repression of a  MATa1 reporter gene when juxtaposed between the gene and the silencer, and its deletion from the natural chromosome leads to a 60% reduction of expression of the downstream  GIT1 gene ( ).	gene_phenotype
71905	4	333982	5	NULL	NULL	0	NULL	HMR-tRNA	NucleicAcid		is juxtaposed between					silencer	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_32_17_5206_s_142	15459290	We have previously shown that the  HMR-tRNA ( tRNA Thr [AGU] CR1) acts as a barrier to the spread of silencing at the  HMR locus, as it blocks repression of a  MATa1 reporter gene when juxtaposed between the gene and the silencer, and its deletion from the natural chromosome leads to a 60% reduction of expression of the downstream  GIT1 gene ( ).	gene_phenotype
71906	5	333982	5	NULL	NULL	0	NULL	statement 3	Process		occurs along with					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_32_17_5206_s_142	15459290	We have previously shown that the  HMR-tRNA ( tRNA Thr [AGU] CR1) acts as a barrier to the spread of silencing at the  HMR locus, as it blocks repression of a  MATa1 reporter gene when juxtaposed between the gene and the silencer, and its deletion from the natural chromosome leads to a 60% reduction of expression of the downstream  GIT1 gene ( ).	gene_phenotype
71907	6	333982	5	NULL	NULL	0	NULL	statement 5	Process		leads to					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_32_17_5206_s_142	15459290	We have previously shown that the  HMR-tRNA ( tRNA Thr [AGU] CR1) acts as a barrier to the spread of silencing at the  HMR locus, as it blocks repression of a  MATa1 reporter gene when juxtaposed between the gene and the silencer, and its deletion from the natural chromosome leads to a 60% reduction of expression of the downstream  GIT1 gene ( ).	gene_phenotype
71908	7	333982	5	NULL	NULL	0	NULL	silencing	Process		occurs at					HMR locus	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_32_17_5206_s_142	15459290	We have previously shown that the  HMR-tRNA ( tRNA Thr [AGU] CR1) acts as a barrier to the spread of silencing at the  HMR locus, as it blocks repression of a  MATa1 reporter gene when juxtaposed between the gene and the silencer, and its deletion from the natural chromosome leads to a 60% reduction of expression of the downstream  GIT1 gene ( ).	gene_phenotype
71909	8	333982	5	NULL	NULL	0	NULL	HMR-tRNA	NucleicAcid		is a barrier to					statement 7	Process	spread of			NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_32_17_5206_s_142	15459290	We have previously shown that the  HMR-tRNA ( tRNA Thr [AGU] CR1) acts as a barrier to the spread of silencing at the  HMR locus, as it blocks repression of a  MATa1 reporter gene when juxtaposed between the gene and the silencer, and its deletion from the natural chromosome leads to a 60% reduction of expression of the downstream  GIT1 gene ( ).	gene_phenotype
71910	9	333982	5	NULL	NULL	0	NULL	HMR-tRNA	NucleicAcid	deletion of	reduce					GIT1 gene	GP	expression of;;downstream			NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_32_17_5206_s_142	15459290	We have previously shown that the  HMR-tRNA ( tRNA Thr [AGU] CR1) acts as a barrier to the spread of silencing at the  HMR locus, as it blocks repression of a  MATa1 reporter gene when juxtaposed between the gene and the silencer, and its deletion from the natural chromosome leads to a 60% reduction of expression of the downstream  GIT1 gene ( ).	gene_phenotype
71911	10	333982	5	NULL	NULL	0	NULL	HMR-tRNA	NucleicAcid		is					tRNA Thr [AGU] CR1	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_32_17_5206_s_142	15459290	We have previously shown that the  HMR-tRNA ( tRNA Thr [AGU] CR1) acts as a barrier to the spread of silencing at the  HMR locus, as it blocks repression of a  MATa1 reporter gene when juxtaposed between the gene and the silencer, and its deletion from the natural chromosome leads to a 60% reduction of expression of the downstream  GIT1 gene ( ).	gene_phenotype
71079	1	333984	5	NULL	NULL	NULL	NULL	snR190	NucleicAcid		is a type of					snoRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_13_3726_s_3	9649442	We show that the snR190 and U14 snoRNAs from the yeast  Saccharomyces cerevisiae are co-transcribed as a dicistronic precursor which is processed by the RNA endonuclease Rnt1, the yeast ortholog of bacterial RNase III.  RNT1 disruption results in a dramatic decrease in the levels of mature U14 and snR190 and in accumulation of dicistronic snR190-U14 RNAs.	gene_phenotype
71080	2	333984	5	NULL	NULL	NULL	NULL	U14	NucleicAcid		is a type of					snoRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_embo_17_13_3726_s_3	9649442	We show that the snR190 and U14 snoRNAs from the yeast  Saccharomyces cerevisiae are co-transcribed as a dicistronic precursor which is processed by the RNA endonuclease Rnt1, the yeast ortholog of bacterial RNase III.  RNT1 disruption results in a dramatic decrease in the levels of mature U14 and snR190 and in accumulation of dicistronic snR190-U14 RNAs.	gene_phenotype
71081	3	333984	5	NULL	NULL	0	NULL	snR190	NucleicAcid	Saccharomyces cerevisiae	is co-transcribed with					U14	NucleicAcid	Saccharomyces cerevisiae			NULL		0	NULL	NULL	NULL	gw60_embo_17_13_3726_s_3	9649442	We show that the snR190 and U14 snoRNAs from the yeast  Saccharomyces cerevisiae are co-transcribed as a dicistronic precursor which is processed by the RNA endonuclease Rnt1, the yeast ortholog of bacterial RNase III.  RNT1 disruption results in a dramatic decrease in the levels of mature U14 and snR190 and in accumulation of dicistronic snR190-U14 RNAs.	gene_phenotype
71082	4	333984	5	NULL	NULL	0	NULL	statement 3	Process		occurs as					dicistronic precursor	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_embo_17_13_3726_s_3	9649442	We show that the snR190 and U14 snoRNAs from the yeast  Saccharomyces cerevisiae are co-transcribed as a dicistronic precursor which is processed by the RNA endonuclease Rnt1, the yeast ortholog of bacterial RNase III.  RNT1 disruption results in a dramatic decrease in the levels of mature U14 and snR190 and in accumulation of dicistronic snR190-U14 RNAs.	gene_phenotype
71083	5	333984	5	NULL	NULL	0	NULL	Rnt1	GP		is a type of					RNA endonuclease	GP				NULL		0	NULL	NULL	NULL	gw60_embo_17_13_3726_s_3	9649442	We show that the snR190 and U14 snoRNAs from the yeast  Saccharomyces cerevisiae are co-transcribed as a dicistronic precursor which is processed by the RNA endonuclease Rnt1, the yeast ortholog of bacterial RNase III.  RNT1 disruption results in a dramatic decrease in the levels of mature U14 and snR190 and in accumulation of dicistronic snR190-U14 RNAs.	gene_phenotype
71084	6	333984	5	NULL	NULL	NULL	NULL	dicistronic precursor	NucleicAcid		is processed by					Rnt1	GP	yeast			NULL		NULL	NULL	NULL	NULL	gw60_embo_17_13_3726_s_3	9649442	We show that the snR190 and U14 snoRNAs from the yeast  Saccharomyces cerevisiae are co-transcribed as a dicistronic precursor which is processed by the RNA endonuclease Rnt1, the yeast ortholog of bacterial RNase III.  RNT1 disruption results in a dramatic decrease in the levels of mature U14 and snR190 and in accumulation of dicistronic snR190-U14 RNAs.	gene_phenotype
71085	7	333984	5	NULL	NULL	0	NULL	Rnt1	GP	yeast	is an orthologue of					RNase III	GP	bacteria			NULL		0	NULL	NULL	NULL	gw60_embo_17_13_3726_s_3	9649442	We show that the snR190 and U14 snoRNAs from the yeast  Saccharomyces cerevisiae are co-transcribed as a dicistronic precursor which is processed by the RNA endonuclease Rnt1, the yeast ortholog of bacterial RNase III.  RNT1 disruption results in a dramatic decrease in the levels of mature U14 and snR190 and in accumulation of dicistronic snR190-U14 RNAs.	gene_phenotype
71087	8	333984	5	NULL	NULL	0	NULL	RNT1	GP	disruption of	decreases		dramatically			U14	NucleicAcid	levels of;;mature			NULL		0	NULL	NULL	NULL	gw60_embo_17_13_3726_s_3	9649442	We show that the snR190 and U14 snoRNAs from the yeast  Saccharomyces cerevisiae are co-transcribed as a dicistronic precursor which is processed by the RNA endonuclease Rnt1, the yeast ortholog of bacterial RNase III.  RNT1 disruption results in a dramatic decrease in the levels of mature U14 and snR190 and in accumulation of dicistronic snR190-U14 RNAs.	gene_phenotype
71088	9	333984	5	NULL	NULL	0	NULL	RNT1	GP	disruption of	decreases		dramatically			snR190	NucleicAcid	levels of;;mature			NULL		0	NULL	NULL	NULL	gw60_embo_17_13_3726_s_3	9649442	We show that the snR190 and U14 snoRNAs from the yeast  Saccharomyces cerevisiae are co-transcribed as a dicistronic precursor which is processed by the RNA endonuclease Rnt1, the yeast ortholog of bacterial RNase III.  RNT1 disruption results in a dramatic decrease in the levels of mature U14 and snR190 and in accumulation of dicistronic snR190-U14 RNAs.	gene_phenotype
71089	10	333984	5	NULL	NULL	0	NULL	RNT1	GP	disruption of	decreases		dramatically			snR190-U14 RNAs	NucleicAcid	accumulation of;;dicistronic			NULL		0	NULL	NULL	NULL	gw60_embo_17_13_3726_s_3	9649442	We show that the snR190 and U14 snoRNAs from the yeast  Saccharomyces cerevisiae are co-transcribed as a dicistronic precursor which is processed by the RNA endonuclease Rnt1, the yeast ortholog of bacterial RNase III.  RNT1 disruption results in a dramatic decrease in the levels of mature U14 and snR190 and in accumulation of dicistronic snR190-U14 RNAs.	gene_phenotype
71107	1	333987	5	NULL	NULL	0	NULL	Rnt1	GP		cleaves					dicistronic RNAs	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_embo_17_13_3726_s_159	9649442	The ability of recombinant Rnt1 to chase the endogenous dicistronic RNAs into mature U14 and snR190 in  rnt1delta extracts, and the accumulation of 5''-extended forms of U14 and snR190 in the  rat1 and  xrn1 exonuclease mutants (Petfalski  et al., 1998  ) suggest a pathway in which the dicistronic RNAs are first cleaved by Rnt1 and then processed to the mature ends by exonucleases which are present in the extract.	gene_phenotype
71108	2	333987	5	NULL	NULL	0	NULL	exonucleases	GP		process					dicistronic RNAs	NucleicAcid	cleaved			NULL		0	NULL	NULL	NULL	gw60_embo_17_13_3726_s_159	9649442	The ability of recombinant Rnt1 to chase the endogenous dicistronic RNAs into mature U14 and snR190 in  rnt1delta extracts, and the accumulation of 5''-extended forms of U14 and snR190 in the  rat1 and  xrn1 exonuclease mutants (Petfalski  et al., 1998  ) suggest a pathway in which the dicistronic RNAs are first cleaved by Rnt1 and then processed to the mature ends by exonucleases which are present in the extract.	gene_phenotype
71109	3	333987	5	NULL	NULL	0	NULL	statement 1	Process		is followed by					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_embo_17_13_3726_s_159	9649442	The ability of recombinant Rnt1 to chase the endogenous dicistronic RNAs into mature U14 and snR190 in  rnt1delta extracts, and the accumulation of 5''-extended forms of U14 and snR190 in the  rat1 and  xrn1 exonuclease mutants (Petfalski  et al., 1998  ) suggest a pathway in which the dicistronic RNAs are first cleaved by Rnt1 and then processed to the mature ends by exonucleases which are present in the extract.	gene_phenotype
71110	1	333988	5	NULL	NULL	0	NULL	Rcl1p	GP	depletion of	affects		possibly			snoRNAs	NucleicAcid	accumulation of			NULL		0	NULL	NULL	NULL	gw60_embo_19_9_2115_s_172	10790377	We therefore investigated whether depletion of Rcl1p affects the accumulation of these or other snoRNAs; the snoRNAs investigated included some transcribed from independent genes as monomeric (U3, snR10 and snR30) or dimeric (U14 and snR190) RNAs, or processed from introns (U24) (reviewed by  Maxwell and Fournier, 1995;  Tollervey and Kiss, 1997).	gene_phenotype
71111	1	333989	5	NULL	NULL	0	NULL	UMOs	NucleicAcid		is a type of					co-linear DNA sequence	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_embo_17_13_3726_s_99	9649442	These probes gave rise to protected bands of the same size as snR190 and U14 snoRNAs in RNAs from the wild-type cells, and of the same size as the UMOs species from the  rnt1delta cells (data not shown), indicating that the UMOs are co-linear with the DNA sequence and that they do not arise from a splicing or a genomic rearrangement event.	gene_phenotype
71112	2	333989	5	NULL	NULL	0	NULL	UMOs	NucleicAcid		does not arise from					splicing	Process				NULL		0	NULL	NULL	NULL	gw60_embo_17_13_3726_s_99	9649442	These probes gave rise to protected bands of the same size as snR190 and U14 snoRNAs in RNAs from the wild-type cells, and of the same size as the UMOs species from the  rnt1delta cells (data not shown), indicating that the UMOs are co-linear with the DNA sequence and that they do not arise from a splicing or a genomic rearrangement event.	gene_phenotype
71113	3	333989	5	NULL	NULL	0	NULL	UMOs	NucleicAcid		does not arise from					genomic rearrangement event	Process				NULL		0	NULL	NULL	NULL	gw60_embo_17_13_3726_s_99	9649442	These probes gave rise to protected bands of the same size as snR190 and U14 snoRNAs in RNAs from the wild-type cells, and of the same size as the UMOs species from the  rnt1delta cells (data not shown), indicating that the UMOs are co-linear with the DNA sequence and that they do not arise from a splicing or a genomic rearrangement event.	gene_phenotype
71114	4	333989	5	NULL	NULL	0	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_embo_17_13_3726_s_99	9649442	These probes gave rise to protected bands of the same size as snR190 and U14 snoRNAs in RNAs from the wild-type cells, and of the same size as the UMOs species from the  rnt1delta cells (data not shown), indicating that the UMOs are co-linear with the DNA sequence and that they do not arise from a splicing or a genomic rearrangement event.	gene_phenotype
71115	1	333990	5	NULL	NULL	0	NULL	U14	NucleicAcid		is essential for					cell viability	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_12_7897_s_238	10567516	However, the snR190-U14 precursor probably retains at least some functionality, since U14 is essential for cell viability and depletion of U14 does block pre-rRNA processing at sites A1 and A2 ( 113).	gene_phenotype
71116	2	333990	5	NULL	NULL	0	NULL	U14	NucleicAcid	depletion of	block					pre-rRNA	NucleicAcid	processing of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_12_7897_s_238	10567516	However, the snR190-U14 precursor probably retains at least some functionality, since U14 is essential for cell viability and depletion of U14 does block pre-rRNA processing at sites A1 and A2 ( 113).	gene_phenotype
71117	1	333992	5	NULL	NULL	0	NULL	NME1	GP	S. cerevisiae	is necessary for					viability	Process				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_66_0_409_s_136	9242913	Cloning of the  S. cerevisiae gene encoding the RNA component of RNase MRP ( NME1) revealed that it is necessary for viability, consistent with an essential nuclear  function ( 50).	gene_phenotype
71118	2	333992	5	NULL	NULL	0	NULL	NME1	GP	S. cerevisiae	is essential for					nuclear function	Process				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_66_0_409_s_136	9242913	Cloning of the  S. cerevisiae gene encoding the RNA component of RNase MRP ( NME1) revealed that it is necessary for viability, consistent with an essential nuclear  function ( 50).	gene_phenotype
71119	3	333992	5	NULL	NULL	NULL	NULL	NME1	GP	S. cerevisiae	is RNA component of					MRP	GP	S.cerevisiae			NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_66_0_409_s_136	9242913	Cloning of the  S. cerevisiae gene encoding the RNA component of RNase MRP ( NME1) revealed that it is necessary for viability, consistent with an essential nuclear  function ( 50).	gene_phenotype
71120	4	333992	5	NULL	NULL	0	NULL	MRP	GP		is a type of					RNase	GP				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_66_0_409_s_136	9242913	Cloning of the  S. cerevisiae gene encoding the RNA component of RNase MRP ( NME1) revealed that it is necessary for viability, consistent with an essential nuclear  function ( 50).	gene_phenotype
71121	1	333994	5	NULL	NULL	0	NULL	hc PUS4	GP	presence of	accumulates					tRNA precursors	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_7_2505_s_6	10713174	The presence of hc PUS4 or hc NME1 led to the accumulation of certain tRNA precursors, and their Gcd  phenotypes were reversed by overexpressing the RNA component of RNase P ( RPR1), responsible for 5''-end processing of all tRNAs.	gene_phenotype
71122	2	333994	5	NULL	NULL	0	NULL	hc NME1	GP	presence of	accumulates					tRNA precursors	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_7_2505_s_6	10713174	The presence of hc PUS4 or hc NME1 led to the accumulation of certain tRNA precursors, and their Gcd  phenotypes were reversed by overexpressing the RNA component of RNase P ( RPR1), responsible for 5''-end processing of all tRNAs.	gene_phenotype
71123	3	333994	5	NULL	NULL	0	NULL	RPR1	GP		is responsible for					tRNAs	NucleicAcid	5''-end processing of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_7_2505_s_6	10713174	The presence of hc PUS4 or hc NME1 led to the accumulation of certain tRNA precursors, and their Gcd  phenotypes were reversed by overexpressing the RNA component of RNase P ( RPR1), responsible for 5''-end processing of all tRNAs.	gene_phenotype
71124	4	333994	5	NULL	NULL	NULL	NULL	RPR1	GP	overexpression of	reverse					Gcd phenotypes	PhysicalPhenomenon				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_7_2505_s_6	10713174	The presence of hc PUS4 or hc NME1 led to the accumulation of certain tRNA precursors, and their Gcd  phenotypes were reversed by overexpressing the RNA component of RNase P ( RPR1), responsible for 5''-end processing of all tRNAs.	gene_phenotype
71125	5	333994	5	NULL	NULL	0	NULL	RPR1	GP		is RNA component of					RNase P	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_7_2505_s_6	10713174	The presence of hc PUS4 or hc NME1 led to the accumulation of certain tRNA precursors, and their Gcd  phenotypes were reversed by overexpressing the RNA component of RNase P ( RPR1), responsible for 5''-end processing of all tRNAs.	gene_phenotype
71182	1	333995	5	NULL	NULL	0	NULL	RMRP	GP	mutation	is introduced into					NME1	GP	yeast			NULL		0	NULL	NULL	NULL	abs-batch0540-0549_hum-mol-genet_14_23_16254002_s_7	16254002	RMRP mutations introduced into  the yeast ortholog, NME1, exhibited normal mitochondrial function, chromosomal  segregation and cell cycle progression, while a CHH fibroblast cell line  exhibited normal mitochondrial content.	gene_phenotype
71183	2	333995	5	NULL	NULL	0	NULL	statement 1	Process		exhibit					mitochondria	CellComponent	normal function of			NULL		0	NULL	NULL	NULL	abs-batch0540-0549_hum-mol-genet_14_23_16254002_s_7	16254002	RMRP mutations introduced into  the yeast ortholog, NME1, exhibited normal mitochondrial function, chromosomal  segregation and cell cycle progression, while a CHH fibroblast cell line  exhibited normal mitochondrial content.	gene_phenotype
71186	3	333995	5	NULL	NULL	0	NULL	statement 1	Process		exhibit					chromosome	Chromosome	normal segregation of			NULL		0	NULL	NULL	NULL	abs-batch0540-0549_hum-mol-genet_14_23_16254002_s_7	16254002	RMRP mutations introduced into  the yeast ortholog, NME1, exhibited normal mitochondrial function, chromosomal  segregation and cell cycle progression, while a CHH fibroblast cell line  exhibited normal mitochondrial content.	gene_phenotype
71188	4	333995	5	NULL	NULL	0	NULL	statement 1	Process		exhibit					cell cycle	Process	normal progression of			NULL		0	NULL	NULL	NULL	abs-batch0540-0549_hum-mol-genet_14_23_16254002_s_7	16254002	RMRP mutations introduced into  the yeast ortholog, NME1, exhibited normal mitochondrial function, chromosomal  segregation and cell cycle progression, while a CHH fibroblast cell line  exhibited normal mitochondrial content.	gene_phenotype
71189	5	333995	5	NULL	NULL	0	NULL	CHH	Cell		is a type of					fibroblast cell line	Cell				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_hum-mol-genet_14_23_16254002_s_7	16254002	RMRP mutations introduced into  the yeast ortholog, NME1, exhibited normal mitochondrial function, chromosomal  segregation and cell cycle progression, while a CHH fibroblast cell line  exhibited normal mitochondrial content.	gene_phenotype
71190	6	333995	5	NULL	NULL	0	NULL	CHH	Cell		exhibit					mitochondria	CellComponent	normal content of			NULL		0	NULL	NULL	NULL	abs-batch0540-0549_hum-mol-genet_14_23_16254002_s_7	16254002	RMRP mutations introduced into  the yeast ortholog, NME1, exhibited normal mitochondrial function, chromosomal  segregation and cell cycle progression, while a CHH fibroblast cell line  exhibited normal mitochondrial content.	gene_phenotype
71192	1	333996	5	NULL	NULL	0	NULL	GCN4 mRNA	NucleicAcid	translation of	is induced by					NME1	GP	overexpression of			NULL		0	NULL	NULL	NULL	gw70_genesdev_17_2_162_s_103	12533506	Thus,  GCN4 mRNA translation can be induced by overexpression of either  NME1, encoding the RNA subunit of RNase MRP (Tavernarakis et al. 1996 ), or of  PUS4, encoding psi55 pseudouridylase (Qiu et al. 2000 ), and both phenotypes are correlated with increased accumulation of pre-tRNAs.	gene_phenotype
71194	2	333996	5	NULL	NULL	NULL	NULL	NME1	GP		encodes for					RNA subunit of MRP	GP				NULL		NULL	NULL	NULL	NULL	gw70_genesdev_17_2_162_s_103	12533506	Thus,  GCN4 mRNA translation can be induced by overexpression of either  NME1, encoding the RNA subunit of RNase MRP (Tavernarakis et al. 1996 ), or of  PUS4, encoding psi55 pseudouridylase (Qiu et al. 2000 ), and both phenotypes are correlated with increased accumulation of pre-tRNAs.	gene_phenotype
71195	3	333996	5	NULL	NULL	0	NULL	MRP	GP		is a type of					RNase	GP				NULL		0	NULL	NULL	NULL	gw70_genesdev_17_2_162_s_103	12533506	Thus,  GCN4 mRNA translation can be induced by overexpression of either  NME1, encoding the RNA subunit of RNase MRP (Tavernarakis et al. 1996 ), or of  PUS4, encoding psi55 pseudouridylase (Qiu et al. 2000 ), and both phenotypes are correlated with increased accumulation of pre-tRNAs.	gene_phenotype
71196	4	333996	5	NULL	NULL	0	NULL	GCN4 mRNA	NucleicAcid	translation of	is induced by					PUS4	GP	overexpression of			NULL		0	NULL	NULL	NULL	gw70_genesdev_17_2_162_s_103	12533506	Thus,  GCN4 mRNA translation can be induced by overexpression of either  NME1, encoding the RNA subunit of RNase MRP (Tavernarakis et al. 1996 ), or of  PUS4, encoding psi55 pseudouridylase (Qiu et al. 2000 ), and both phenotypes are correlated with increased accumulation of pre-tRNAs.	gene_phenotype
71197	5	333996	5	NULL	NULL	0	NULL	PUS4	GP		encodes for					psi55 pseudouridylase 	GP				NULL		0	NULL	NULL	NULL	gw70_genesdev_17_2_162_s_103	12533506	Thus,  GCN4 mRNA translation can be induced by overexpression of either  NME1, encoding the RNA subunit of RNase MRP (Tavernarakis et al. 1996 ), or of  PUS4, encoding psi55 pseudouridylase (Qiu et al. 2000 ), and both phenotypes are correlated with increased accumulation of pre-tRNAs.	gene_phenotype
71198	1	333997	5	NULL	NULL	0	NULL	PCNA	GP		plays a role in		putative			metastasis	Process				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_arch-otolaryngol-head-neck-surg_123_4_9109790_s_11	9109790	The following markers were selected on their  putative role in the process of metastasis and were studied using immunohistochemical  and/or Southern blot techniques: proliferating cell nuclear antigen (PCNA),  p53, retinoblastoma tumor-suppressor gene (Rb), myc, bcl-2 (inhibitor  of apoptosis), epidermal growth factor (EGF), EGF-receptor (EGFR), neu,  nm23 (also known as NME1, putative metastasis suppressor), desmoplakin,  neuron cell-adhesion molecule (N-CAM), epithelial cell-adhesion molecule  (Ep-CAM), E-cadherin, cyclin D1 (CCND1), and EMS1.	gene_phenotype
71199	2	333997	5	NULL	NULL	0	NULL	p53	GP		plays a role in		putative			metastasis	Process				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_arch-otolaryngol-head-neck-surg_123_4_9109790_s_11	9109790	The following markers were selected on their  putative role in the process of metastasis and were studied using immunohistochemical  and/or Southern blot techniques: proliferating cell nuclear antigen (PCNA),  p53, retinoblastoma tumor-suppressor gene (Rb), myc, bcl-2 (inhibitor  of apoptosis), epidermal growth factor (EGF), EGF-receptor (EGFR), neu,  nm23 (also known as NME1, putative metastasis suppressor), desmoplakin,  neuron cell-adhesion molecule (N-CAM), epithelial cell-adhesion molecule  (Ep-CAM), E-cadherin, cyclin D1 (CCND1), and EMS1.	gene_phenotype
71200	3	333997	5	NULL	NULL	0	NULL	Rb	GP		plays a role in		putative			metastasis	Process				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_arch-otolaryngol-head-neck-surg_123_4_9109790_s_11	9109790	The following markers were selected on their  putative role in the process of metastasis and were studied using immunohistochemical  and/or Southern blot techniques: proliferating cell nuclear antigen (PCNA),  p53, retinoblastoma tumor-suppressor gene (Rb), myc, bcl-2 (inhibitor  of apoptosis), epidermal growth factor (EGF), EGF-receptor (EGFR), neu,  nm23 (also known as NME1, putative metastasis suppressor), desmoplakin,  neuron cell-adhesion molecule (N-CAM), epithelial cell-adhesion molecule  (Ep-CAM), E-cadherin, cyclin D1 (CCND1), and EMS1.	gene_phenotype
71201	4	333997	5	NULL	NULL	0	NULL	myc	GP		plays a role in		putative			metastasis	Process				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_arch-otolaryngol-head-neck-surg_123_4_9109790_s_11	9109790	The following markers were selected on their  putative role in the process of metastasis and were studied using immunohistochemical  and/or Southern blot techniques: proliferating cell nuclear antigen (PCNA),  p53, retinoblastoma tumor-suppressor gene (Rb), myc, bcl-2 (inhibitor  of apoptosis), epidermal growth factor (EGF), EGF-receptor (EGFR), neu,  nm23 (also known as NME1, putative metastasis suppressor), desmoplakin,  neuron cell-adhesion molecule (N-CAM), epithelial cell-adhesion molecule  (Ep-CAM), E-cadherin, cyclin D1 (CCND1), and EMS1.	gene_phenotype
71202	5	333997	5	NULL	NULL	0	NULL	bcl-2	GP		plays a role in		putative			metastasis	Process				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_arch-otolaryngol-head-neck-surg_123_4_9109790_s_11	9109790	The following markers were selected on their  putative role in the process of metastasis and were studied using immunohistochemical  and/or Southern blot techniques: proliferating cell nuclear antigen (PCNA),  p53, retinoblastoma tumor-suppressor gene (Rb), myc, bcl-2 (inhibitor  of apoptosis), epidermal growth factor (EGF), EGF-receptor (EGFR), neu,  nm23 (also known as NME1, putative metastasis suppressor), desmoplakin,  neuron cell-adhesion molecule (N-CAM), epithelial cell-adhesion molecule  (Ep-CAM), E-cadherin, cyclin D1 (CCND1), and EMS1.	gene_phenotype
71203	6	333997	5	NULL	NULL	0	NULL	EGF	GP		plays a role in		putative			metastasis	Process				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_arch-otolaryngol-head-neck-surg_123_4_9109790_s_11	9109790	The following markers were selected on their  putative role in the process of metastasis and were studied using immunohistochemical  and/or Southern blot techniques: proliferating cell nuclear antigen (PCNA),  p53, retinoblastoma tumor-suppressor gene (Rb), myc, bcl-2 (inhibitor  of apoptosis), epidermal growth factor (EGF), EGF-receptor (EGFR), neu,  nm23 (also known as NME1, putative metastasis suppressor), desmoplakin,  neuron cell-adhesion molecule (N-CAM), epithelial cell-adhesion molecule  (Ep-CAM), E-cadherin, cyclin D1 (CCND1), and EMS1.	gene_phenotype
71204	7	333997	5	NULL	NULL	0	NULL	EGFR	GP		plays a role in		putative			metastasis	Process				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_arch-otolaryngol-head-neck-surg_123_4_9109790_s_11	9109790	The following markers were selected on their  putative role in the process of metastasis and were studied using immunohistochemical  and/or Southern blot techniques: proliferating cell nuclear antigen (PCNA),  p53, retinoblastoma tumor-suppressor gene (Rb), myc, bcl-2 (inhibitor  of apoptosis), epidermal growth factor (EGF), EGF-receptor (EGFR), neu,  nm23 (also known as NME1, putative metastasis suppressor), desmoplakin,  neuron cell-adhesion molecule (N-CAM), epithelial cell-adhesion molecule  (Ep-CAM), E-cadherin, cyclin D1 (CCND1), and EMS1.	gene_phenotype
71205	8	333997	5	NULL	NULL	0	NULL	neu	GP		plays a role in		putative			metastasis	Process				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_arch-otolaryngol-head-neck-surg_123_4_9109790_s_11	9109790	The following markers were selected on their  putative role in the process of metastasis and were studied using immunohistochemical  and/or Southern blot techniques: proliferating cell nuclear antigen (PCNA),  p53, retinoblastoma tumor-suppressor gene (Rb), myc, bcl-2 (inhibitor  of apoptosis), epidermal growth factor (EGF), EGF-receptor (EGFR), neu,  nm23 (also known as NME1, putative metastasis suppressor), desmoplakin,  neuron cell-adhesion molecule (N-CAM), epithelial cell-adhesion molecule  (Ep-CAM), E-cadherin, cyclin D1 (CCND1), and EMS1.	gene_phenotype
71206	9	333997	5	NULL	NULL	0	NULL	nm23	GP		plays a role in		putative			metastasis	Process				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_arch-otolaryngol-head-neck-surg_123_4_9109790_s_11	9109790	The following markers were selected on their  putative role in the process of metastasis and were studied using immunohistochemical  and/or Southern blot techniques: proliferating cell nuclear antigen (PCNA),  p53, retinoblastoma tumor-suppressor gene (Rb), myc, bcl-2 (inhibitor  of apoptosis), epidermal growth factor (EGF), EGF-receptor (EGFR), neu,  nm23 (also known as NME1, putative metastasis suppressor), desmoplakin,  neuron cell-adhesion molecule (N-CAM), epithelial cell-adhesion molecule  (Ep-CAM), E-cadherin, cyclin D1 (CCND1), and EMS1.	gene_phenotype
71207	10	333997	5	NULL	NULL	0	NULL	desmoplakin	GP		plays a role in		putative			metastasis	Process				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_arch-otolaryngol-head-neck-surg_123_4_9109790_s_11	9109790	The following markers were selected on their  putative role in the process of metastasis and were studied using immunohistochemical  and/or Southern blot techniques: proliferating cell nuclear antigen (PCNA),  p53, retinoblastoma tumor-suppressor gene (Rb), myc, bcl-2 (inhibitor  of apoptosis), epidermal growth factor (EGF), EGF-receptor (EGFR), neu,  nm23 (also known as NME1, putative metastasis suppressor), desmoplakin,  neuron cell-adhesion molecule (N-CAM), epithelial cell-adhesion molecule  (Ep-CAM), E-cadherin, cyclin D1 (CCND1), and EMS1.	gene_phenotype
71208	11	333997	5	NULL	NULL	0	NULL	N-CAM	GP		plays a role in		putative			metastasis	Process				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_arch-otolaryngol-head-neck-surg_123_4_9109790_s_11	9109790	The following markers were selected on their  putative role in the process of metastasis and were studied using immunohistochemical  and/or Southern blot techniques: proliferating cell nuclear antigen (PCNA),  p53, retinoblastoma tumor-suppressor gene (Rb), myc, bcl-2 (inhibitor  of apoptosis), epidermal growth factor (EGF), EGF-receptor (EGFR), neu,  nm23 (also known as NME1, putative metastasis suppressor), desmoplakin,  neuron cell-adhesion molecule (N-CAM), epithelial cell-adhesion molecule  (Ep-CAM), E-cadherin, cyclin D1 (CCND1), and EMS1.	gene_phenotype
71209	12	333997	5	NULL	NULL	0	NULL	Ep-CAM	GP		plays a role in		putative			metastasis	Process				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_arch-otolaryngol-head-neck-surg_123_4_9109790_s_11	9109790	The following markers were selected on their  putative role in the process of metastasis and were studied using immunohistochemical  and/or Southern blot techniques: proliferating cell nuclear antigen (PCNA),  p53, retinoblastoma tumor-suppressor gene (Rb), myc, bcl-2 (inhibitor  of apoptosis), epidermal growth factor (EGF), EGF-receptor (EGFR), neu,  nm23 (also known as NME1, putative metastasis suppressor), desmoplakin,  neuron cell-adhesion molecule (N-CAM), epithelial cell-adhesion molecule  (Ep-CAM), E-cadherin, cyclin D1 (CCND1), and EMS1.	gene_phenotype
71210	13	333997	5	NULL	NULL	0	NULL	E-cadherin	GP		plays a role in		putative			metastasis	Process				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_arch-otolaryngol-head-neck-surg_123_4_9109790_s_11	9109790	The following markers were selected on their  putative role in the process of metastasis and were studied using immunohistochemical  and/or Southern blot techniques: proliferating cell nuclear antigen (PCNA),  p53, retinoblastoma tumor-suppressor gene (Rb), myc, bcl-2 (inhibitor  of apoptosis), epidermal growth factor (EGF), EGF-receptor (EGFR), neu,  nm23 (also known as NME1, putative metastasis suppressor), desmoplakin,  neuron cell-adhesion molecule (N-CAM), epithelial cell-adhesion molecule  (Ep-CAM), E-cadherin, cyclin D1 (CCND1), and EMS1.	gene_phenotype
71211	14	333997	5	NULL	NULL	NULL	NULL	CCND1	GP		plays a role in		putative			metastasis	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_arch-otolaryngol-head-neck-surg_123_4_9109790_s_11	9109790	The following markers were selected on their  putative role in the process of metastasis and were studied using immunohistochemical  and/or Southern blot techniques: proliferating cell nuclear antigen (PCNA),  p53, retinoblastoma tumor-suppressor gene (Rb), myc, bcl-2 (inhibitor  of apoptosis), epidermal growth factor (EGF), EGF-receptor (EGFR), neu,  nm23 (also known as NME1, putative metastasis suppressor), desmoplakin,  neuron cell-adhesion molecule (N-CAM), epithelial cell-adhesion molecule  (Ep-CAM), E-cadherin, cyclin D1 (CCND1), and EMS1.	gene_phenotype
71212	15	333997	5	NULL	NULL	0	NULL	EMS1	GP		plays a role in		putative			metastasis	Process				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_arch-otolaryngol-head-neck-surg_123_4_9109790_s_11	9109790	The following markers were selected on their  putative role in the process of metastasis and were studied using immunohistochemical  and/or Southern blot techniques: proliferating cell nuclear antigen (PCNA),  p53, retinoblastoma tumor-suppressor gene (Rb), myc, bcl-2 (inhibitor  of apoptosis), epidermal growth factor (EGF), EGF-receptor (EGFR), neu,  nm23 (also known as NME1, putative metastasis suppressor), desmoplakin,  neuron cell-adhesion molecule (N-CAM), epithelial cell-adhesion molecule  (Ep-CAM), E-cadherin, cyclin D1 (CCND1), and EMS1.	gene_phenotype
71213	16	333997	5	NULL	NULL	0	NULL	PCNA	GP		is					proliferating cell nuclear antigen	GP				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_arch-otolaryngol-head-neck-surg_123_4_9109790_s_11	9109790	The following markers were selected on their  putative role in the process of metastasis and were studied using immunohistochemical  and/or Southern blot techniques: proliferating cell nuclear antigen (PCNA),  p53, retinoblastoma tumor-suppressor gene (Rb), myc, bcl-2 (inhibitor  of apoptosis), epidermal growth factor (EGF), EGF-receptor (EGFR), neu,  nm23 (also known as NME1, putative metastasis suppressor), desmoplakin,  neuron cell-adhesion molecule (N-CAM), epithelial cell-adhesion molecule  (Ep-CAM), E-cadherin, cyclin D1 (CCND1), and EMS1.	gene_phenotype
71214	17	333997	5	NULL	NULL	0	NULL	Rb	GP		is					retinoblastoma tumor-suppressor gene	GP				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_arch-otolaryngol-head-neck-surg_123_4_9109790_s_11	9109790	The following markers were selected on their  putative role in the process of metastasis and were studied using immunohistochemical  and/or Southern blot techniques: proliferating cell nuclear antigen (PCNA),  p53, retinoblastoma tumor-suppressor gene (Rb), myc, bcl-2 (inhibitor  of apoptosis), epidermal growth factor (EGF), EGF-receptor (EGFR), neu,  nm23 (also known as NME1, putative metastasis suppressor), desmoplakin,  neuron cell-adhesion molecule (N-CAM), epithelial cell-adhesion molecule  (Ep-CAM), E-cadherin, cyclin D1 (CCND1), and EMS1.	gene_phenotype
71215	18	333997	5	NULL	NULL	0	NULL	bcl-2	GP		is an inhibitor of					apoptosis	Process				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_arch-otolaryngol-head-neck-surg_123_4_9109790_s_11	9109790	The following markers were selected on their  putative role in the process of metastasis and were studied using immunohistochemical  and/or Southern blot techniques: proliferating cell nuclear antigen (PCNA),  p53, retinoblastoma tumor-suppressor gene (Rb), myc, bcl-2 (inhibitor  of apoptosis), epidermal growth factor (EGF), EGF-receptor (EGFR), neu,  nm23 (also known as NME1, putative metastasis suppressor), desmoplakin,  neuron cell-adhesion molecule (N-CAM), epithelial cell-adhesion molecule  (Ep-CAM), E-cadherin, cyclin D1 (CCND1), and EMS1.	gene_phenotype
71216	19	333997	5	NULL	NULL	0	NULL	EGF	GP		is					epidermal growth factor	GP				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_arch-otolaryngol-head-neck-surg_123_4_9109790_s_11	9109790	The following markers were selected on their  putative role in the process of metastasis and were studied using immunohistochemical  and/or Southern blot techniques: proliferating cell nuclear antigen (PCNA),  p53, retinoblastoma tumor-suppressor gene (Rb), myc, bcl-2 (inhibitor  of apoptosis), epidermal growth factor (EGF), EGF-receptor (EGFR), neu,  nm23 (also known as NME1, putative metastasis suppressor), desmoplakin,  neuron cell-adhesion molecule (N-CAM), epithelial cell-adhesion molecule  (Ep-CAM), E-cadherin, cyclin D1 (CCND1), and EMS1.	gene_phenotype
71217	20	333997	5	NULL	NULL	0	NULL	EGFR	GP		is					EGF-receptor	GP				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_arch-otolaryngol-head-neck-surg_123_4_9109790_s_11	9109790	The following markers were selected on their  putative role in the process of metastasis and were studied using immunohistochemical  and/or Southern blot techniques: proliferating cell nuclear antigen (PCNA),  p53, retinoblastoma tumor-suppressor gene (Rb), myc, bcl-2 (inhibitor  of apoptosis), epidermal growth factor (EGF), EGF-receptor (EGFR), neu,  nm23 (also known as NME1, putative metastasis suppressor), desmoplakin,  neuron cell-adhesion molecule (N-CAM), epithelial cell-adhesion molecule  (Ep-CAM), E-cadherin, cyclin D1 (CCND1), and EMS1.	gene_phenotype
71224	21	333997	5	NULL	NULL	0	NULL	NME1	GP		is a synonym of					nm23	GP				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_arch-otolaryngol-head-neck-surg_123_4_9109790_s_11	9109790	The following markers were selected on their  putative role in the process of metastasis and were studied using immunohistochemical  and/or Southern blot techniques: proliferating cell nuclear antigen (PCNA),  p53, retinoblastoma tumor-suppressor gene (Rb), myc, bcl-2 (inhibitor  of apoptosis), epidermal growth factor (EGF), EGF-receptor (EGFR), neu,  nm23 (also known as NME1, putative metastasis suppressor), desmoplakin,  neuron cell-adhesion molecule (N-CAM), epithelial cell-adhesion molecule  (Ep-CAM), E-cadherin, cyclin D1 (CCND1), and EMS1.	gene_phenotype
71225	22	333997	5	NULL	NULL	0	NULL	NME1	GP		is a suppressor of		putative			metastasis	Process				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_arch-otolaryngol-head-neck-surg_123_4_9109790_s_11	9109790	The following markers were selected on their  putative role in the process of metastasis and were studied using immunohistochemical  and/or Southern blot techniques: proliferating cell nuclear antigen (PCNA),  p53, retinoblastoma tumor-suppressor gene (Rb), myc, bcl-2 (inhibitor  of apoptosis), epidermal growth factor (EGF), EGF-receptor (EGFR), neu,  nm23 (also known as NME1, putative metastasis suppressor), desmoplakin,  neuron cell-adhesion molecule (N-CAM), epithelial cell-adhesion molecule  (Ep-CAM), E-cadherin, cyclin D1 (CCND1), and EMS1.	gene_phenotype
71226	23	333997	5	NULL	NULL	0	NULL	N-CAM	GP		is					neuron cell-adhesion molecule	GP				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_arch-otolaryngol-head-neck-surg_123_4_9109790_s_11	9109790	The following markers were selected on their  putative role in the process of metastasis and were studied using immunohistochemical  and/or Southern blot techniques: proliferating cell nuclear antigen (PCNA),  p53, retinoblastoma tumor-suppressor gene (Rb), myc, bcl-2 (inhibitor  of apoptosis), epidermal growth factor (EGF), EGF-receptor (EGFR), neu,  nm23 (also known as NME1, putative metastasis suppressor), desmoplakin,  neuron cell-adhesion molecule (N-CAM), epithelial cell-adhesion molecule  (Ep-CAM), E-cadherin, cyclin D1 (CCND1), and EMS1.	gene_phenotype
71227	24	333997	5	NULL	NULL	0	NULL	Ep-CAM	GP		is					epithelial cell-adhesion molecule	GP				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_arch-otolaryngol-head-neck-surg_123_4_9109790_s_11	9109790	The following markers were selected on their  putative role in the process of metastasis and were studied using immunohistochemical  and/or Southern blot techniques: proliferating cell nuclear antigen (PCNA),  p53, retinoblastoma tumor-suppressor gene (Rb), myc, bcl-2 (inhibitor  of apoptosis), epidermal growth factor (EGF), EGF-receptor (EGFR), neu,  nm23 (also known as NME1, putative metastasis suppressor), desmoplakin,  neuron cell-adhesion molecule (N-CAM), epithelial cell-adhesion molecule  (Ep-CAM), E-cadherin, cyclin D1 (CCND1), and EMS1.	gene_phenotype
71228	25	333997	5	NULL	NULL	0	NULL	CCND1	GP		is					cyclin D1	GP				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_arch-otolaryngol-head-neck-surg_123_4_9109790_s_11	9109790	The following markers were selected on their  putative role in the process of metastasis and were studied using immunohistochemical  and/or Southern blot techniques: proliferating cell nuclear antigen (PCNA),  p53, retinoblastoma tumor-suppressor gene (Rb), myc, bcl-2 (inhibitor  of apoptosis), epidermal growth factor (EGF), EGF-receptor (EGFR), neu,  nm23 (also known as NME1, putative metastasis suppressor), desmoplakin,  neuron cell-adhesion molecule (N-CAM), epithelial cell-adhesion molecule  (Ep-CAM), E-cadherin, cyclin D1 (CCND1), and EMS1.	gene_phenotype
71229	1	333999	5	NULL	NULL	0	NULL	snR10	GP	loss of	impairs					protein synthesis	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_11_2_425_s_237	12620230	Loss of snR10 itself impairs protein synthesis activity, and this defect is not rescued by expression of the snR10 C gene   (Figure 6C).	gene_phenotype
71230	2	333999	5	NULL	NULL	0	NULL	snR10 C gene	GP	expression of	does not rescue					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_11_2_425_s_237	12620230	Loss of snR10 itself impairs protein synthesis activity, and this defect is not rescued by expression of the snR10 C gene   (Figure 6C).	gene_phenotype
71231	1	334000	5	NULL	NULL	0	NULL	U14	NucleicAcid		plays a role in		possibly			rRNA	NucleicAcid	modifying the folding of			NULL		0	NULL	NULL	NULL	gw70_annurevgenet_33_0_261_s_221	10690410	It may be that U14, snR10, and snR30/U17 are derived from conventional modification  guide RNAs but have assumed roles in modifying the folding of the rRNA.	gene_phenotype
71232	2	334000	5	NULL	NULL	0	NULL	snR10	GP		plays a role in		possibly			rRNA	NucleicAcid	modifying the folding of			NULL		0	NULL	NULL	NULL	gw70_annurevgenet_33_0_261_s_221	10690410	It may be that U14, snR10, and snR30/U17 are derived from conventional modification  guide RNAs but have assumed roles in modifying the folding of the rRNA.	gene_phenotype
71233	3	334000	5	NULL	NULL	0	NULL	snR30/U17	NucleicAcid		plays a role in		possibly			rRNA	NucleicAcid	modifying the folding of			NULL		0	NULL	NULL	NULL	gw70_annurevgenet_33_0_261_s_221	10690410	It may be that U14, snR10, and snR30/U17 are derived from conventional modification  guide RNAs but have assumed roles in modifying the folding of the rRNA.	gene_phenotype
71246	1	334001	5	NULL	NULL	0	NULL	SNR10	NucleicAcid		is a type of					H/ACA small RNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_pnas_103_11_4192_s_60	16537507	( a)  SNR10 is a 245-bases-long essential H/ACA small RNA required for modification of rRNA precursor  sequence.	gene_phenotype
71247	2	334001	5	NULL	NULL	0	NULL	SNR10	GP		is required for					rRNA precursor sequence	NucleicAcid	modification of			NULL		0	NULL	NULL	NULL	gw70_pnas_103_11_4192_s_60	16537507	( a)  SNR10 is a 245-bases-long essential H/ACA small RNA required for modification of rRNA precursor  sequence.	gene_phenotype
71248	1	334002	5	NULL	NULL	0	NULL	snR30	NucleicAcid		is required for					cell viability	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_4_1769_s_38	14749391	While yeast cells lacking snR10 are only slightly impaired in cell growth and in processing of 35S pre-rRNA, snR30 is essential for cell viability ( ,  ).	gene_phenotype
71249	2	334002	5	NULL	NULL	0	NULL	yeast cells	Cell		lacks					snR10	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_4_1769_s_38	14749391	While yeast cells lacking snR10 are only slightly impaired in cell growth and in processing of 35S pre-rRNA, snR30 is essential for cell viability ( ,  ).	gene_phenotype
71250	3	334002	5	NULL	NULL	0	NULL	statement 2	Cell		impaired in		slightly			cell growth	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_4_1769_s_38	14749391	While yeast cells lacking snR10 are only slightly impaired in cell growth and in processing of 35S pre-rRNA, snR30 is essential for cell viability ( ,  ).	gene_phenotype
71251	4	334002	5	NULL	NULL	0	NULL	statement 2	Cell		impaired in		slightly			35S pre-rRNA	NucleicAcid	processing of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_4_1769_s_38	14749391	While yeast cells lacking snR10 are only slightly impaired in cell growth and in processing of 35S pre-rRNA, snR30 is essential for cell viability ( ,  ).	gene_phenotype
71252	1	334003	5	NULL	NULL	0	NULL	snoRNAs	NucleicAcid		is required for					rRNA	NucleicAcid	modification of			NULL		0	NULL	NULL	NULL	gw60_genesdev_12_4_527_s_30	9472021	In contrast, none of the snoRNAs that direct rRNA modification is essential for cell viability, although the absence of the   guide snoRNA, snR10, leads to some cold sensitivity (Tollervey 1987  ; Ni et al. 1997  ).	gene_phenotype
71253	2	334003	5	NULL	NULL	0	NULL	statement 1	Process		is not essential for					cell viability	Process				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_4_527_s_30	9472021	In contrast, none of the snoRNAs that direct rRNA modification is essential for cell viability, although the absence of the   guide snoRNA, snR10, leads to some cold sensitivity (Tollervey 1987  ; Ni et al. 1997  ).	gene_phenotype
71254	3	334003	5	NULL	NULL	0	NULL	snR10	NucleicAcid	absence of	leads to					cold sensitivity	Process				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_4_527_s_30	9472021	In contrast, none of the snoRNAs that direct rRNA modification is essential for cell viability, although the absence of the   guide snoRNA, snR10, leads to some cold sensitivity (Tollervey 1987  ; Ni et al. 1997  ).	gene_phenotype
71255	4	334003	5	NULL	NULL	0	NULL	snR10	NucleicAcid		is a type of					guide snoRNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_4_527_s_30	9472021	In contrast, none of the snoRNAs that direct rRNA modification is essential for cell viability, although the absence of the   guide snoRNA, snR10, leads to some cold sensitivity (Tollervey 1987  ; Ni et al. 1997  ).	gene_phenotype
71256	1	334004	5	NULL	NULL	0	NULL	snR30	NucleicAcid		is a type of					box H/ACA snoRNAs	NucleicAcid				NULL	yeast	0	NULL	NULL	NULL	gw60_cellbiol_144_6_1123_s_322	10087258	This is not surprising, given that all  box H/ACA snoRNAs found in yeast, with the exception of snR30 (Morrissey and Tollervey, 1993  ) and snR10 (Tollervey, 1987  ; Tollervey and Guthrie, 1985  ), are dispensable for viability.	gene_phenotype
71257	2	334004	5	NULL	NULL	0	NULL	snR10	NucleicAcid		is a type of					box H/ACA snoRNAs	NucleicAcid				NULL	yeast	0	NULL	NULL	NULL	gw60_cellbiol_144_6_1123_s_322	10087258	This is not surprising, given that all  box H/ACA snoRNAs found in yeast, with the exception of snR30 (Morrissey and Tollervey, 1993  ) and snR10 (Tollervey, 1987  ; Tollervey and Guthrie, 1985  ), are dispensable for viability.	gene_phenotype
71258	3	334004	5	NULL	NULL	0	NULL	box H/ACA snoRNAs	NucleicAcid		is dispensable for					viability	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_144_6_1123_s_322	10087258	This is not surprising, given that all  box H/ACA snoRNAs found in yeast, with the exception of snR30 (Morrissey and Tollervey, 1993  ) and snR10 (Tollervey, 1987  ; Tollervey and Guthrie, 1985  ), are dispensable for viability.	gene_phenotype
71259	4	334004	5	NULL	NULL	0	NULL	snR10	NucleicAcid		is not dispensable for					viability					NULL		0	NULL	NULL	NULL	gw60_cellbiol_144_6_1123_s_322	10087258	This is not surprising, given that all  box H/ACA snoRNAs found in yeast, with the exception of snR30 (Morrissey and Tollervey, 1993  ) and snR10 (Tollervey, 1987  ; Tollervey and Guthrie, 1985  ), are dispensable for viability.	gene_phenotype
71260	5	334004	5	NULL	NULL	0	NULL	snR30	NucleicAcid		is not dispensable for					viability	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_144_6_1123_s_322	10087258	This is not surprising, given that all  box H/ACA snoRNAs found in yeast, with the exception of snR30 (Morrissey and Tollervey, 1993  ) and snR10 (Tollervey, 1987  ; Tollervey and Guthrie, 1985  ), are dispensable for viability.	gene_phenotype
71261	1	334005	5	NULL	NULL	0	NULL	snR10	GP		influences					18S RNA	NucleicAcid	production of			NULL		0	NULL	NULL	NULL	gw60_molcell_11_2_425_s_192	12620230	Because snR10 also influences production of 18S RNA and accumulation of 40S subunits, it is important to determine if the defects observed in growth and ribosome activity are due to loss of the  2919 modification or impaired processing of 18S rRNA.	gene_phenotype
71262	2	334005	5	NULL	NULL	0	NULL	snR10	NucleicAcid		influences					40S subunits	NucleicAcid	accumulation of			NULL		0	NULL	NULL	NULL	gw60_molcell_11_2_425_s_192	12620230	Because snR10 also influences production of 18S RNA and accumulation of 40S subunits, it is important to determine if the defects observed in growth and ribosome activity are due to loss of the  2919 modification or impaired processing of 18S rRNA.	gene_phenotype
71900	2	334007	5	NULL	NULL	0	NULL	RXR-TR heterodimer	GP	obligate	mediates					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_6_3375_s_77	9452457	Thus T-CoR repressed gene activation mediated by an obligate RXR-TR heterodimer from the sub-optimal TRE 6DR4.	gene_phenotype
71901	1	334007	5	NULL	NULL	NULL	NULL	gene activation	Process		is repressed by					T-CoR	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_6_3375_s_77	9452457	Thus T-CoR repressed gene activation mediated by an obligate RXR-TR heterodimer from the sub-optimal TRE 6DR4.	gene_phenotype
71263	1	334008	5	NULL	NULL	0	NULL	snR10	NucleicAcid		is essential for					rRNA	NucleicAcid	processing of			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_10_11_3877_s_24	10564278	Some snoRNAs of the box H/ACA family are essential for rRNA processing (snR10 [Tollervey, 1987  ], snR30 [Morrissey and Tollervey, 1993  ], and E1 = U17, E2, and E3 [Mishra and Elicieri, 1997  ]), but the majority function as guide RNAs for pseudouridine modifications in rRNA (Ganot  et al., 1997a  ; Ni  et al., 1997  ; Smith and Steitz, 1997  ).	gene_phenotype
71264	2	334008	5	NULL	NULL	0	NULL	snR30	NucleicAcid		is essential for					rRNA	NucleicAcid	processing of			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_10_11_3877_s_24	10564278	Some snoRNAs of the box H/ACA family are essential for rRNA processing (snR10 [Tollervey, 1987  ], snR30 [Morrissey and Tollervey, 1993  ], and E1 = U17, E2, and E3 [Mishra and Elicieri, 1997  ]), but the majority function as guide RNAs for pseudouridine modifications in rRNA (Ganot  et al., 1997a  ; Ni  et al., 1997  ; Smith and Steitz, 1997  ).	gene_phenotype
71265	3	334008	5	NULL	NULL	0	NULL	E1	NucleicAcid		is essential for					rRNA	NucleicAcid	processing of			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_10_11_3877_s_24	10564278	Some snoRNAs of the box H/ACA family are essential for rRNA processing (snR10 [Tollervey, 1987  ], snR30 [Morrissey and Tollervey, 1993  ], and E1 = U17, E2, and E3 [Mishra and Elicieri, 1997  ]), but the majority function as guide RNAs for pseudouridine modifications in rRNA (Ganot  et al., 1997a  ; Ni  et al., 1997  ; Smith and Steitz, 1997  ).	gene_phenotype
71266	4	334008	5	NULL	NULL	0	NULL	snR10	NucleicAcid		is a member of					box H/ACA family of snoRNAs 	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_10_11_3877_s_24	10564278	Some snoRNAs of the box H/ACA family are essential for rRNA processing (snR10 [Tollervey, 1987  ], snR30 [Morrissey and Tollervey, 1993  ], and E1 = U17, E2, and E3 [Mishra and Elicieri, 1997  ]), but the majority function as guide RNAs for pseudouridine modifications in rRNA (Ganot  et al., 1997a  ; Ni  et al., 1997  ; Smith and Steitz, 1997  ).	gene_phenotype
71267	5	334008	5	NULL	NULL	0	NULL	snR30	NucleicAcid		is a member of					box H/ACA family of snoRNAs	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_10_11_3877_s_24	10564278	Some snoRNAs of the box H/ACA family are essential for rRNA processing (snR10 [Tollervey, 1987  ], snR30 [Morrissey and Tollervey, 1993  ], and E1 = U17, E2, and E3 [Mishra and Elicieri, 1997  ]), but the majority function as guide RNAs for pseudouridine modifications in rRNA (Ganot  et al., 1997a  ; Ni  et al., 1997  ; Smith and Steitz, 1997  ).	gene_phenotype
71268	6	334008	5	NULL	NULL	0	NULL	E1 	NucleicAcid		is a member of					box H/ACA family of snoRNAs	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_10_11_3877_s_24	10564278	Some snoRNAs of the box H/ACA family are essential for rRNA processing (snR10 [Tollervey, 1987  ], snR30 [Morrissey and Tollervey, 1993  ], and E1 = U17, E2, and E3 [Mishra and Elicieri, 1997  ]), but the majority function as guide RNAs for pseudouridine modifications in rRNA (Ganot  et al., 1997a  ; Ni  et al., 1997  ; Smith and Steitz, 1997  ).	gene_phenotype
71269	7	334008	5	NULL	NULL	0	NULL	box H/ACA family of snoRNAs	NucleicAcid	majority of	functions as					guide RNAs	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_10_11_3877_s_24	10564278	Some snoRNAs of the box H/ACA family are essential for rRNA processing (snR10 [Tollervey, 1987  ], snR30 [Morrissey and Tollervey, 1993  ], and E1 = U17, E2, and E3 [Mishra and Elicieri, 1997  ]), but the majority function as guide RNAs for pseudouridine modifications in rRNA (Ganot  et al., 1997a  ; Ni  et al., 1997  ; Smith and Steitz, 1997  ).	gene_phenotype
71270	8	334008	5	NULL	NULL	0	NULL	guide RNAs	NucleicAcid		is required for					rRNA	NucleicAcid	pseudouridine modifications of			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_10_11_3877_s_24	10564278	Some snoRNAs of the box H/ACA family are essential for rRNA processing (snR10 [Tollervey, 1987  ], snR30 [Morrissey and Tollervey, 1993  ], and E1 = U17, E2, and E3 [Mishra and Elicieri, 1997  ]), but the majority function as guide RNAs for pseudouridine modifications in rRNA (Ganot  et al., 1997a  ; Ni  et al., 1997  ; Smith and Steitz, 1997  ).	gene_phenotype
71271	1	334014	5	NULL	NULL	0	NULL	cold sensitivity	Process	suppression of	involves		may			PET494	GP	stimulation of;;transcription of			NULL		0	NULL	NULL	NULL	gw70_yeast_20_11_955_s_418	12898711	As no sequence changes distinguishing  PET494 from the wild-type allele were found, the suppression of the cold sensitivity seemed  to involve stimulation of the  PET494 transcription.	gene_phenotype
71878	1	334022	5	NULL	NULL	0	NULL	PET54	GP		is an activator of					translation	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_4_1826_s_104	9528754	The wild-type function of the  COX3-specific translational activators  PET54,  PET122, and  PET494 was required for respiratory growth of the  cox3-15 strains carrying  MRP21 or  MRP51 suppressor alleles.	gene_phenotype
71879	2	334022	5	NULL	NULL	0	NULL	statement 1	Process		is specific to					COX3	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_4_1826_s_104	9528754	The wild-type function of the  COX3-specific translational activators  PET54,  PET122, and  PET494 was required for respiratory growth of the  cox3-15 strains carrying  MRP21 or  MRP51 suppressor alleles.	gene_phenotype
71881	3	334022	5	NULL	NULL	0	NULL	PET122	GP		is an activator of					translation	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_4_1826_s_104	9528754	The wild-type function of the  COX3-specific translational activators  PET54,  PET122, and  PET494 was required for respiratory growth of the  cox3-15 strains carrying  MRP21 or  MRP51 suppressor alleles.	gene_phenotype
71883	4	334022	5	NULL	NULL	0	NULL	statement 1	Process		is specific to					COX3	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_4_1826_s_104	9528754	The wild-type function of the  COX3-specific translational activators  PET54,  PET122, and  PET494 was required for respiratory growth of the  cox3-15 strains carrying  MRP21 or  MRP51 suppressor alleles.	gene_phenotype
71884	5	334022	5	NULL	NULL	0	NULL	PET494	GP		is an activator of					translation	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_4_1826_s_104	9528754	The wild-type function of the  COX3-specific translational activators  PET54,  PET122, and  PET494 was required for respiratory growth of the  cox3-15 strains carrying  MRP21 or  MRP51 suppressor alleles.	gene_phenotype
71885	6	334022	5	NULL	NULL	0	NULL	statement 1	Process		is specific to					COX3	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_4_1826_s_104	9528754	The wild-type function of the  COX3-specific translational activators  PET54,  PET122, and  PET494 was required for respiratory growth of the  cox3-15 strains carrying  MRP21 or  MRP51 suppressor alleles.	gene_phenotype
71886	7	334022	5	NULL	NULL	0	NULL	cox3-15 strain	Organism		carry					MRP21	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_4_1826_s_104	9528754	The wild-type function of the  COX3-specific translational activators  PET54,  PET122, and  PET494 was required for respiratory growth of the  cox3-15 strains carrying  MRP21 or  MRP51 suppressor alleles.	gene_phenotype
71887	8	334022	5	NULL	NULL	0	NULL	cox3-15 strain	Organism		carry					MRP51	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_4_1826_s_104	9528754	The wild-type function of the  COX3-specific translational activators  PET54,  PET122, and  PET494 was required for respiratory growth of the  cox3-15 strains carrying  MRP21 or  MRP51 suppressor alleles.	gene_phenotype
71888	9	334022	5	NULL	NULL	0	NULL	statement 7	Process		is an alternative to					statement 8	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_4_1826_s_104	9528754	The wild-type function of the  COX3-specific translational activators  PET54,  PET122, and  PET494 was required for respiratory growth of the  cox3-15 strains carrying  MRP21 or  MRP51 suppressor alleles.	gene_phenotype
71889	10	334022	5	NULL	NULL	0	NULL	MRP21	GP		is a type of					suppressor allele	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_4_1826_s_104	9528754	The wild-type function of the  COX3-specific translational activators  PET54,  PET122, and  PET494 was required for respiratory growth of the  cox3-15 strains carrying  MRP21 or  MRP51 suppressor alleles.	gene_phenotype
71890	11	334022	5	NULL	NULL	0	NULL	MRP51	GP		is a type of					suppressor allele	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_4_1826_s_104	9528754	The wild-type function of the  COX3-specific translational activators  PET54,  PET122, and  PET494 was required for respiratory growth of the  cox3-15 strains carrying  MRP21 or  MRP51 suppressor alleles.	gene_phenotype
71891	12	334022	5	NULL	NULL	0	NULL	PET54	GP	wild-type function of	is required for					statement 7	Process	respiratory growth of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_4_1826_s_104	9528754	The wild-type function of the  COX3-specific translational activators  PET54,  PET122, and  PET494 was required for respiratory growth of the  cox3-15 strains carrying  MRP21 or  MRP51 suppressor alleles.	gene_phenotype
71893	13	334022	5	NULL	NULL	NULL	NULL	PET54	GP	wild-type function of	is required for					statement 8	Process	respiratory growth of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_4_1826_s_104	9528754	The wild-type function of the  COX3-specific translational activators  PET54,  PET122, and  PET494 was required for respiratory growth of the  cox3-15 strains carrying  MRP21 or  MRP51 suppressor alleles.	gene_phenotype
71895	14	334022	5	NULL	NULL	0	NULL	PET122	GP	wild-type function of	is required for					statement 7	Process	respiratory growth of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_4_1826_s_104	9528754	The wild-type function of the  COX3-specific translational activators  PET54,  PET122, and  PET494 was required for respiratory growth of the  cox3-15 strains carrying  MRP21 or  MRP51 suppressor alleles.	gene_phenotype
71897	15	334022	5	NULL	NULL	0	NULL	PET122	GP	wild-type function of	is required for					statement 8	Process	respiratory growth of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_4_1826_s_104	9528754	The wild-type function of the  COX3-specific translational activators  PET54,  PET122, and  PET494 was required for respiratory growth of the  cox3-15 strains carrying  MRP21 or  MRP51 suppressor alleles.	gene_phenotype
71898	16	334022	5	NULL	NULL	0	NULL	PET494	GP	wild-type function of	is required for					statement 7	Process	respiratory growth of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_4_1826_s_104	9528754	The wild-type function of the  COX3-specific translational activators  PET54,  PET122, and  PET494 was required for respiratory growth of the  cox3-15 strains carrying  MRP21 or  MRP51 suppressor alleles.	gene_phenotype
71899	17	334022	5	NULL	NULL	0	NULL	PET494	GP	wild-type function of	is required for					statement 8	Process	respiratory growth of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_4_1826_s_104	9528754	The wild-type function of the  COX3-specific translational activators  PET54,  PET122, and  PET494 was required for respiratory growth of the  cox3-15 strains carrying  MRP21 or  MRP51 suppressor alleles.	gene_phenotype
69692	1	334026	7	NULL	NULL	0	NULL	R30m1 cells	Cell		does not grow on					glucose-containing medium	Chemical				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_4_1769_s_187	14749391	In contrast to the efficient expression of snR30m1 and snR30m2, neither the  R30m1 nor the  R30m2 cells could grow on glucose-containing medium (Fig.  6C), demonstrating that the m1 and m2 motifs of snR30, although not required for RNA accumulation, are essential for cell viability.	gene_phenotype
69693	2	334026	7	NULL	NULL	0	NULL	R30m2 cells	Cell		does not grow on					glucose-containing medium	Chemical				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_4_1769_s_187	14749391	In contrast to the efficient expression of snR30m1 and snR30m2, neither the  R30m1 nor the  R30m2 cells could grow on glucose-containing medium (Fig.  6C), demonstrating that the m1 and m2 motifs of snR30, although not required for RNA accumulation, are essential for cell viability.	gene_phenotype
69694	3	334026	7	NULL	NULL	0	NULL	snR30	NucleicAcid		not required for			m1 motif		RNA	NucleicAcid	accumulation of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_4_1769_s_187	14749391	In contrast to the efficient expression of snR30m1 and snR30m2, neither the  R30m1 nor the  R30m2 cells could grow on glucose-containing medium (Fig.  6C), demonstrating that the m1 and m2 motifs of snR30, although not required for RNA accumulation, are essential for cell viability.	gene_phenotype
69695	4	334026	7	NULL	NULL	0	NULL	snR30	NucleicAcid		not required for			m2 motif		RNA	NucleicAcid	accumulation of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_4_1769_s_187	14749391	In contrast to the efficient expression of snR30m1 and snR30m2, neither the  R30m1 nor the  R30m2 cells could grow on glucose-containing medium (Fig.  6C), demonstrating that the m1 and m2 motifs of snR30, although not required for RNA accumulation, are essential for cell viability.	gene_phenotype
69696	5	334026	7	NULL	NULL	0	NULL	snR30	NucleicAcid		is essential for			m1 motif		cell viability	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_4_1769_s_187	14749391	In contrast to the efficient expression of snR30m1 and snR30m2, neither the  R30m1 nor the  R30m2 cells could grow on glucose-containing medium (Fig.  6C), demonstrating that the m1 and m2 motifs of snR30, although not required for RNA accumulation, are essential for cell viability.	gene_phenotype
69697	6	334026	7	NULL	NULL	0	NULL	snR30	NucleicAcid		is essential for			m2 motif		cell viability	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_4_1769_s_187	14749391	In contrast to the efficient expression of snR30m1 and snR30m2, neither the  R30m1 nor the  R30m2 cells could grow on glucose-containing medium (Fig.  6C), demonstrating that the m1 and m2 motifs of snR30, although not required for RNA accumulation, are essential for cell viability.	gene_phenotype
69762	1	334027	7	NULL	NULL	0	NULL	yeast cells	Cell		express					snR30m2	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_4_1769_s_253	14749391	Moreover, we have recently found that the viability of yeast cells expressing snR30m2, but not snR30m1, could be restored by coexpression of the human U17a snoRNA (our unpublished data).	gene_phenotype
69763	2	334027	7	NULL	NULL	0	NULL	statement 1	Process	viability of	restored by					U17a snoRNA	NucleicAcid	coexpression of;;human			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_4_1769_s_253	14749391	Moreover, we have recently found that the viability of yeast cells expressing snR30m2, but not snR30m1, could be restored by coexpression of the human U17a snoRNA (our unpublished data).	gene_phenotype
69767	1	334028	7	NULL	NULL	0	NULL	cell viability elements	Chemical		located in the					snR30	NucleicAcid			3' hairpin	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_4_1769_s_104	14749391	Elements essential for cell viability are located in the 3' hairpin of snR30.	gene_phenotype
69768	1	334029	7	NULL	NULL	0	NULL	snR30	NucleicAcid		essential for			 conserved m1 element		cell viability	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_4_1769_s_189	14749391	The conserved m1 and m2 elements of snR30 are essential for cell viability.	gene_phenotype
69777	2	334029	7	NULL	NULL	NULL	NULL	snR30	NucleicAcid		essential for			conserved m2 element		cell viability	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_4_1769_s_189	14749391	The conserved m1 and m2 elements of snR30 are essential for cell viability.	gene_phenotype
69778	1	334030	7	NULL	NULL	0	NULL	R5-R30S chimeric RNA 	NucleicAcid		support					cell growth	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_4_1769_s_143	14749391	In conclusion, the results of the deletion analysis of snR30, taken together with the finding that R5-R30S chimeric RNA can support cell growth, indicate that all the elements essential for cell viability are contained within the 3''-terminal hairpin of snR30.	gene_phenotype
69779	2	334030	7	NULL	NULL	0	NULL	cell viability elements	Chemical		contained within					snR30	NucleicAcid		3''-terminal hairpin		NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_4_1769_s_143	14749391	In conclusion, the results of the deletion analysis of snR30, taken together with the finding that R5-R30S chimeric RNA can support cell growth, indicate that all the elements essential for cell viability are contained within the 3''-terminal hairpin of snR30.	gene_phenotype
69780	3	334030	7	NULL	NULL	0	NULL	statement 1	Process		indicate					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_4_1769_s_143	14749391	In conclusion, the results of the deletion analysis of snR30, taken together with the finding that R5-R30S chimeric RNA can support cell growth, indicate that all the elements essential for cell viability are contained within the 3''-terminal hairpin of snR30.	gene_phenotype
69781	1	334031	7	NULL	NULL	0	NULL	 snR30	NucleicAcid	yeast	required for					18S rRNA	NucleicAcid	production of			NULL		0	NULL	NULL	NULL	gw60_cell_89_5_799_s_31	9182768	Yeast snR30 is required for production of 18S rRNA and, therefore, for cell  viability (Bally et al., 1988   ;  Morrissey and Tollervey, 1993   ).	gene_phenotype
69782	2	334031	7	NULL	NULL	0	NULL	statement 1	Process		required for					cell viability	Process				NULL		0	NULL	NULL	NULL	gw60_cell_89_5_799_s_31	9182768	Yeast snR30 is required for production of 18S rRNA and, therefore, for cell  viability (Bally et al., 1988   ;  Morrissey and Tollervey, 1993   ).	gene_phenotype
69795	1	334032	7	NULL	NULL	0	NULL	snR30 RNA	NucleicAcid	depletion of essential	leads to					 27SA3 pre-rRNA	NucleicAcid	accumulation of			NULL		0	NULL	NULL	NULL	gw60_pnas_97_24_13027_s_229	11087857	Depletion of the essential snR30 RNA, a member of the box H/ACA class of snoRNAs, leads to accumulation of the 27SA3 pre-rRNA ( 6).	gene_phenotype
69796	2	334032	7	NULL	NULL	0	NULL	snR30 RNA	NucleicAcid		is a member of					snoRNA	NucleicAcid			box H/ACA class 	NULL		0	NULL	NULL	NULL	gw60_pnas_97_24_13027_s_229	11087857	Depletion of the essential snR30 RNA, a member of the box H/ACA class of snoRNAs, leads to accumulation of the 27SA3 pre-rRNA ( 6).	gene_phenotype
69797	1	334033	7	NULL	NULL	NULL	NULL	snR30	NucleicAcid	removal of	does not influence				internal hairpin of from U398 to A529	R30-dIH RNA	NucleicAcid	accumulation of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_4_1769_s_115	14749391	Likewise, removal of the internal hairpin of snR30 (from U398 to A529) had no influence on the accumulation of the resulting R30-dIH RNA (Fig.  3D, lane 5).	gene_phenotype
69798	1	334034	7	NULL	NULL	0	NULL	snR30	NucleicAcid		carries				3''-terminal hairpin	cell viability	Process	critical for		elements	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_4_1769_s_230	14749391	Expression of an snR5-snR30 chimeric RNA (R5-R30S) demonstrated that the 3''-terminal hairpin of snR30 carries all the elements that are critical for cell viability (Fig.  3).	gene_phenotype
69799	1	334036	7	NULL	NULL	0	NULL	snR30	NucleicAcid		play critical role in			 m1 motif		cell viability	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_4_1769_s_201	14749391	To test whether the critical role played by the m1 and m2 motifs of snR30 in cell viability is connected to 18S production, the processing of pre-rRNA in the  R30m1 and  R30m2 strains was investigated.	gene_phenotype
69800	2	334036	7	NULL	NULL	0	NULL	snR30	NucleicAcid		play critical role in			m2 motif		cell viability	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_4_1769_s_201	14749391	To test whether the critical role played by the m1 and m2 motifs of snR30 in cell viability is connected to 18S production, the processing of pre-rRNA in the  R30m1 and  R30m2 strains was investigated.	gene_phenotype
69801	1	334037	7	NULL	NULL	0	NULL	H/ACA RNA 	NucleicAcid	trypanosome	involved in					rRNA	NucleicAcid	maturation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_41_34558_s_55	16107339	The first trypanosome H/ACA RNA involved in rRNA maturation, the snR30 homologue, was identified in this study, and the defects in rRNA maturation during CBF5 silencing can be attributed in part to its absence.	gene_phenotype
69802	2	334037	7	NULL	NULL	0	NULL	H/ACA RNA 	NucleicAcid	trypanosome	is a homologue of					snR30	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_41_34558_s_55	16107339	The first trypanosome H/ACA RNA involved in rRNA maturation, the snR30 homologue, was identified in this study, and the defects in rRNA maturation during CBF5 silencing can be attributed in part to its absence.	gene_phenotype
69803	3	334037	7	NULL	NULL	NULL	NULL	rRNA	NucleicAcid	defects in maturation of	is attributed to		partly			H/ACA RNA	NucleicAcid	absence of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_41_34558_s_55	16107339	The first trypanosome H/ACA RNA involved in rRNA maturation, the snR30 homologue, was identified in this study, and the defects in rRNA maturation during CBF5 silencing can be attributed in part to its absence.	gene_phenotype
69804	4	334037	7	NULL	NULL	0	NULL	rRNA	NucleicAcid	defects in maturation of	occur during					CBF5	GP	silencing of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_41_34558_s_55	16107339	The first trypanosome H/ACA RNA involved in rRNA maturation, the snR30 homologue, was identified in this study, and the defects in rRNA maturation during CBF5 silencing can be attributed in part to its absence.	gene_phenotype
69806	1	334038	7	NULL	NULL	NULL	NULL	 snoRNA snR30	NucleicAcid		essential for				box H/ACA	rRNA	NucleicAcid	processing of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_26_23553_s_281	12700234	Because box H/ACA snoRNA snR30 is essential for rRNA  processing and consequently viability of yeast  ( ), its depletion is the  likely cause for growth arrest after Srp40p depletion.	gene_phenotype
69808	2	334038	7	NULL	NULL	NULL	NULL	snoRNA snR30 	NucleicAcid		essential for			 	box H/ACA	viability	Process	yeast			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_26_23553_s_281	12700234	Because box H/ACA snoRNA snR30 is essential for rRNA  processing and consequently viability of yeast  ( ), its depletion is the  likely cause for growth arrest after Srp40p depletion.	gene_phenotype
69809	3	334038	7	NULL	NULL	0	NULL	snoRNA snR30	NucleicAcid	depletion of	cause for				box H/ACA	growth arrest	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_26_23553_s_281	12700234	Because box H/ACA snoRNA snR30 is essential for rRNA  processing and consequently viability of yeast  ( ), its depletion is the  likely cause for growth arrest after Srp40p depletion.	gene_phenotype
69810	4	334038	7	NULL	NULL	0	NULL	statement 3	Process		occur after					Srp40p	GP	depletion of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_26_23553_s_281	12700234	Because box H/ACA snoRNA snR30 is essential for rRNA  processing and consequently viability of yeast  ( ), its depletion is the  likely cause for growth arrest after Srp40p depletion.	gene_phenotype
69811	1	334039	7	NULL	NULL	0	NULL	snoRNA	NucleicAcid	yeast	is required for				box H/ACA	18S rRNA	NucleicAcid	processing of			NULL		0	NULL	NULL	NULL	gw60_embo_16_15_4770_s_27	9303321	All yeast box H/ACA snoRNAs tested, with the exception of snR30 which is required for 18S rRNA processing (Morrissey and Tollervey, 1993  ), are dispensable for viability (Maxwell and Fournier, 1995  ; Balakin  et al., 1996  , and references therein).	gene_phenotype
69814	2	334039	7	NULL	NULL	0	NULL	snR30	NucleicAcid		is not required for					18S rRNA	NucleicAcid	processing of			NULL		0	NULL	NULL	NULL	gw60_embo_16_15_4770_s_27	9303321	All yeast box H/ACA snoRNAs tested, with the exception of snR30 which is required for 18S rRNA processing (Morrissey and Tollervey, 1993  ), are dispensable for viability (Maxwell and Fournier, 1995  ; Balakin  et al., 1996  , and references therein).	gene_phenotype
69815	3	334039	7	NULL	NULL	0	NULL	snoRNA	NucleicAcid	yeast	is dispensable for				box H/ACA	viability	Process				NULL		0	NULL	NULL	NULL	gw60_embo_16_15_4770_s_27	9303321	All yeast box H/ACA snoRNAs tested, with the exception of snR30 which is required for 18S rRNA processing (Morrissey and Tollervey, 1993  ), are dispensable for viability (Maxwell and Fournier, 1995  ; Balakin  et al., 1996  , and references therein).	gene_phenotype
69816	1	334045	7	NULL	NULL	0	NULL	crd1delta	GP	Uncoupled Oxidative Phosphorylation of	is independent of					PET56	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_134	15169766	Uncoupled Oxidative Phosphorylation in crd1delta Is Independent of PET56  -- Mitochondrial function was assayed in  crd1delta mutant cells in the  PET56 genetic background.	gene_phenotype
69817	1	334046	7	NULL	NULL	0	NULL	crd1delta	GP	Coupling in;;mutant	is defective in					PET56 background	GP				NULL	mitochondria	0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_171	15169766	(ii) Coupling and oxidative phosphorylation are defective in  crd1delta mutant mitochondria in  PET56 and  pet56 genetic backgrounds.	gene_phenotype
69818	2	334046	7	NULL	NULL	NULL	NULL	crd1delta	GP	oxidative phosphorylation of;;mutant	is defective in					PET56 background	GP				NULL	mitochondria	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_171	15169766	(ii) Coupling and oxidative phosphorylation are defective in  crd1delta mutant mitochondria in  PET56 and  pet56 genetic backgrounds.	gene_phenotype
69819	3	334046	7	NULL	NULL	NULL	NULL	crd1delta	GP	Coupling in;;mutant	is defective in					pet56 genetic background	GP				NULL	mitochondria	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_171	15169766	(ii) Coupling and oxidative phosphorylation are defective in  crd1delta mutant mitochondria in  PET56 and  pet56 genetic backgrounds.	gene_phenotype
69820	4	334046	7	NULL	NULL	0	NULL	crd1delta	GP	oxidative phosphorylation of;;mutant	is defective in					pet56 genetic background	GP				NULL	mitochondria	0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_171	15169766	(ii) Coupling and oxidative phosphorylation are defective in  crd1delta mutant mitochondria in  PET56 and  pet56 genetic backgrounds.	gene_phenotype
69821	1	334048	7	NULL	NULL	0	NULL	PET56 gene	GP	wild type;;expression of	does not affect					viability	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_107	15169766	Expression of the wild type  PET56 gene did not affect viability.	gene_phenotype
69822	1	334049	7	NULL	NULL	0	NULL	crd1delta	GP	mutant	forms					Petite	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_121	15169766	Increased Petite Formation in crd1delta Mutants at Elevated Temperatures Is Independent of pet56  --	gene_phenotype
69823	2	334049	7	NULL	NULL	0	NULL	temperature		elevated	increase					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_121	15169766	Increased Petite Formation in crd1delta Mutants at Elevated Temperatures Is Independent of pet56  --	gene_phenotype
69824	3	334049	7	NULL	NULL	0	NULL	statement 2	Process		is independent of					pet56	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_121	15169766	Increased Petite Formation in crd1delta Mutants at Elevated Temperatures Is Independent of pet56  --	gene_phenotype
69825	1	334050	7	NULL	NULL	0	NULL	crd1delta	GP	mutant	shows					oxidative phosphorylation	Process	defective			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_142	15169766	The  crd1delta mutant in the  PET56 background exhibits defective oxidative phosphorylation.	gene_phenotype
69826	2	334050	7	NULL	NULL	0	NULL	statement 1	Process		occur in					PET56 background	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_142	15169766	The  crd1delta mutant in the  PET56 background exhibits defective oxidative phosphorylation.	gene_phenotype
69827	1	334051	7	NULL	NULL	NULL	NULL	DNA	NucleicAcid	Decreased viability of;;mitochondrial	occurs at					 temperature		elevated			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_169	15169766	(i) Decreased viability and loss of mitochondrial DNA at elevated temperature are independent of  pet56.	gene_phenotype
69828	2	334051	7	NULL	NULL	0	NULL	DNA	NucleicAcid	loss of;;mitochondrial	occur at					temperature		elevated			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_169	15169766	(i) Decreased viability and loss of mitochondrial DNA at elevated temperature are independent of  pet56.	gene_phenotype
69829	3	334051	7	NULL	NULL	0	NULL	statement 1	Process		is independent of					pet56	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_169	15169766	(i) Decreased viability and loss of mitochondrial DNA at elevated temperature are independent of  pet56.	gene_phenotype
69830	4	334051	7	NULL	NULL	0	NULL	statement 2	Process		is independent of					pet56	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_169	15169766	(i) Decreased viability and loss of mitochondrial DNA at elevated temperature are independent of  pet56.	gene_phenotype
69831	1	334052	7	NULL	NULL	NULL	NULL	crd1delta	GP	viability of;;mutant	is lost upon					pet56 background	GP	growth in			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_105	15169766	The  crd1delta mutant lost viability after prolonged growth in liquid culture (24 and 72 h in  pet56 and  PET56 backgrounds, respectively ( Fig. 3).	gene_phenotype
69832	2	334052	7	NULL	NULL	0	NULL	crd1delta	GP	viability of;;mutant	is lost upon					PET56 background	GP	growth in			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_105	15169766	The  crd1delta mutant lost viability after prolonged growth in liquid culture (24 and 72 h in  pet56 and  PET56 backgrounds, respectively ( Fig. 3).	gene_phenotype
69833	1	334054	7	NULL	NULL	0	NULL	 DL1	GP		shows					mitochondrial function	Process	little			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_102	12840009	Even YPH500 ( pet56) maintained only 40% viability  under these conditions as compared with DL1 and YZD5 ( PET56), which  showed little or no loss of mitochondrial function.	gene_phenotype
69834	2	334054	7	NULL	NULL	0	NULL	YZD5	GP		shows					mitochondrial function	Process	little			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_102	12840009	Even YPH500 ( pet56) maintained only 40% viability  under these conditions as compared with DL1 and YZD5 ( PET56), which  showed little or no loss of mitochondrial function.	gene_phenotype
69835	3	334054	7	NULL	NULL	0	NULL	DL1	GP		shows					mitochondrial function	Process	no loss of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_102	12840009	Even YPH500 ( pet56) maintained only 40% viability  under these conditions as compared with DL1 and YZD5 ( PET56), which  showed little or no loss of mitochondrial function.	gene_phenotype
69836	4	334054	7	NULL	NULL	0	NULL	YZD5	GP		shows					mitochondrial function	Process	no loss of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_102	12840009	Even YPH500 ( pet56) maintained only 40% viability  under these conditions as compared with DL1 and YZD5 ( PET56), which  showed little or no loss of mitochondrial function.	gene_phenotype
69837	5	334054	7	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_102	12840009	Even YPH500 ( pet56) maintained only 40% viability  under these conditions as compared with DL1 and YZD5 ( PET56), which  showed little or no loss of mitochondrial function.	gene_phenotype
69838	6	334054	7	NULL	NULL	0	NULL	statement 2	Process		is an alternative to					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_102	12840009	Even YPH500 ( pet56) maintained only 40% viability  under these conditions as compared with DL1 and YZD5 ( PET56), which  showed little or no loss of mitochondrial function.	gene_phenotype
69839	1	334055	7	NULL	NULL	0	NULL	PET56	GP	reduced expression of	slows					growth	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_25	15169766	Reduced expression of  PET56 was found to slow growth, decrease mitochondrial DNA stability, and decrease cell viability at elevated temperatures ( ,  ).	gene_phenotype
69840	2	334055	7	NULL	NULL	0	NULL	statement 1	Process		occur at					temperature		elevated			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_25	15169766	Reduced expression of  PET56 was found to slow growth, decrease mitochondrial DNA stability, and decrease cell viability at elevated temperatures ( ,  ).	gene_phenotype
69841	3	334055	7	NULL	NULL	0	NULL	PET56	GP	reduced expression of	decrease					DNA	NucleicAcid	stability of;;mitochondrial			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_25	15169766	Reduced expression of  PET56 was found to slow growth, decrease mitochondrial DNA stability, and decrease cell viability at elevated temperatures ( ,  ).	gene_phenotype
69842	4	334055	7	NULL	NULL	0	NULL	statement 3	Process		occur at					temperature		elevated			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_25	15169766	Reduced expression of  PET56 was found to slow growth, decrease mitochondrial DNA stability, and decrease cell viability at elevated temperatures ( ,  ).	gene_phenotype
69843	5	334055	7	NULL	NULL	0	NULL	PET56	GP	reduced expression of	decrease					cell viability	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_25	15169766	Reduced expression of  PET56 was found to slow growth, decrease mitochondrial DNA stability, and decrease cell viability at elevated temperatures ( ,  ).	gene_phenotype
69844	6	334055	7	NULL	NULL	0	NULL	statement 5	Process		occur at					temperature		elevated			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_25	15169766	Reduced expression of  PET56 was found to slow growth, decrease mitochondrial DNA stability, and decrease cell viability at elevated temperatures ( ,  ).	gene_phenotype
69950	1	334056	7	NULL	NULL	0	NULL	 crd1delta	GP		loses					viability	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_115	15169766	Expression of  CRD1 but not  PET56 protects  crd1delta from loss of viability following prolonged culture at elevated temperatures.	gene_phenotype
69951	2	334056	7	NULL	NULL	0	NULL	statement 1	Process		occur at					temperature		elevated			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_115	15169766	Expression of  CRD1 but not  PET56 protects  crd1delta from loss of viability following prolonged culture at elevated temperatures.	gene_phenotype
69952	3	334056	7	NULL	NULL	0	NULL	CRD1	GP	expression of	protects					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_115	15169766	Expression of  CRD1 but not  PET56 protects  crd1delta from loss of viability following prolonged culture at elevated temperatures.	gene_phenotype
69953	4	334056	7	NULL	NULL	0	NULL	PET56	GP	expression of	protects					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_115	15169766	Expression of  CRD1 but not  PET56 protects  crd1delta from loss of viability following prolonged culture at elevated temperatures.	gene_phenotype
69954	1	334057	7	NULL	NULL	NULL	NULL	petite cells 	Cell		present in					crd1delta	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_123	15169766	As seen in  Fig. 4, the percentage of petite cells in the  crd1delta mutant in the  pet56 background was greater than among wild type cells.	gene_phenotype
69955	2	334057	7	NULL	NULL	0	NULL	statement 1	Process		occur in the					pet56 background	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_123	15169766	As seen in  Fig. 4, the percentage of petite cells in the  crd1delta mutant in the  pet56 background was greater than among wild type cells.	gene_phenotype
69956	3	334057	7	NULL	NULL	NULL	NULL	petite cells	Cell		present in					crd1delta 	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_123	15169766	As seen in  Fig. 4, the percentage of petite cells in the  crd1delta mutant in the  pet56 background was greater than among wild type cells.	gene_phenotype
69957	4	334057	7	NULL	NULL	0	NULL	statement 1	Process		is greater than					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_123	15169766	As seen in  Fig. 4, the percentage of petite cells in the  crd1delta mutant in the  pet56 background was greater than among wild type cells.	gene_phenotype
69958	1	334058	7	NULL	NULL	0	NULL	PET56	GP	null mutants	is defective in					mitochondrial large ribosomal subunit	CellComponent	assembly of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_26	12840009	Null mutants in   PET56 are defective in assembly of the mitochondrial large ribosomal  subunit and do not grow on nonfermentable carbon sources, but partial loss of   PET56 expression results in slowed growth, mtDNA instability, and  loss of cell viability at elevated temperatures  ( ,   ) similar to the properties  of  crd1delta strains containing the   his3delta 200 allele  ( ).	gene_phenotype
69959	2	334058	7	NULL	NULL	0	NULL	statement 1	Process		does not grow on					nonfermentable carbon sources	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_26	12840009	Null mutants in   PET56 are defective in assembly of the mitochondrial large ribosomal  subunit and do not grow on nonfermentable carbon sources, but partial loss of   PET56 expression results in slowed growth, mtDNA instability, and  loss of cell viability at elevated temperatures  ( ,   ) similar to the properties  of  crd1delta strains containing the   his3delta 200 allele  ( ).	gene_phenotype
69960	3	334058	7	NULL	NULL	0	NULL	PET56	GP	partial loss of expression of	results in					slowed growth	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_26	12840009	Null mutants in   PET56 are defective in assembly of the mitochondrial large ribosomal  subunit and do not grow on nonfermentable carbon sources, but partial loss of   PET56 expression results in slowed growth, mtDNA instability, and  loss of cell viability at elevated temperatures  ( ,   ) similar to the properties  of  crd1delta strains containing the   his3delta 200 allele  ( ).	gene_phenotype
69961	4	334058	7	NULL	NULL	0	NULL	PET56	GP	partial loss of expression of	results in					 mtDNA	NucleicAcid	instability of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_26	12840009	Null mutants in   PET56 are defective in assembly of the mitochondrial large ribosomal  subunit and do not grow on nonfermentable carbon sources, but partial loss of   PET56 expression results in slowed growth, mtDNA instability, and  loss of cell viability at elevated temperatures  ( ,   ) similar to the properties  of  crd1delta strains containing the   his3delta 200 allele  ( ).	gene_phenotype
69962	5	334058	7	NULL	NULL	0	NULL	PET56	GP	partial loss of expression of	results in					cell viability	Process	loss of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_26	12840009	Null mutants in   PET56 are defective in assembly of the mitochondrial large ribosomal  subunit and do not grow on nonfermentable carbon sources, but partial loss of   PET56 expression results in slowed growth, mtDNA instability, and  loss of cell viability at elevated temperatures  ( ,   ) similar to the properties  of  crd1delta strains containing the   his3delta 200 allele  ( ).	gene_phenotype
69963	6	334058	7	NULL	NULL	0	NULL	statement 3	Process		occur at					temperature		elevated			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_26	12840009	Null mutants in   PET56 are defective in assembly of the mitochondrial large ribosomal  subunit and do not grow on nonfermentable carbon sources, but partial loss of   PET56 expression results in slowed growth, mtDNA instability, and  loss of cell viability at elevated temperatures  ( ,   ) similar to the properties  of  crd1delta strains containing the   his3delta 200 allele  ( ).	gene_phenotype
69964	7	334058	7	NULL	NULL	0	NULL	statement 4	Process		occur at					temperature		elevated			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_26	12840009	Null mutants in   PET56 are defective in assembly of the mitochondrial large ribosomal  subunit and do not grow on nonfermentable carbon sources, but partial loss of   PET56 expression results in slowed growth, mtDNA instability, and  loss of cell viability at elevated temperatures  ( ,   ) similar to the properties  of  crd1delta strains containing the   his3delta 200 allele  ( ).	gene_phenotype
69965	8	334058	7	NULL	NULL	0	NULL	statement 5	Process		occur at					temperature		elevated			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_26	12840009	Null mutants in   PET56 are defective in assembly of the mitochondrial large ribosomal  subunit and do not grow on nonfermentable carbon sources, but partial loss of   PET56 expression results in slowed growth, mtDNA instability, and  loss of cell viability at elevated temperatures  ( ,   ) similar to the properties  of  crd1delta strains containing the   his3delta 200 allele  ( ).	gene_phenotype
69966	9	334058	7	NULL	NULL	0	NULL	crd1delta strains	GP		contain					 his3delta 200 allele	Chromosome				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_26	12840009	Null mutants in   PET56 are defective in assembly of the mitochondrial large ribosomal  subunit and do not grow on nonfermentable carbon sources, but partial loss of   PET56 expression results in slowed growth, mtDNA instability, and  loss of cell viability at elevated temperatures  ( ,   ) similar to the properties  of  crd1delta strains containing the   his3delta 200 allele  ( ).	gene_phenotype
69967	10	334058	7	NULL	NULL	NULL	NULL	statement 9	GP	properties of	similar to					PET56	GP	properties of;; partial loss of expression of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_26	12840009	Null mutants in   PET56 are defective in assembly of the mitochondrial large ribosomal  subunit and do not grow on nonfermentable carbon sources, but partial loss of   PET56 expression results in slowed growth, mtDNA instability, and  loss of cell viability at elevated temperatures  ( ,   ) similar to the properties  of  crd1delta strains containing the   his3delta 200 allele  ( ).	gene_phenotype
69968	1	334059	7	NULL	NULL	NULL	NULL	his3delta 200 allele 	Chromosome	strains containing	shows					 growth	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_89	12840009	Because strains carrying the  his3delta 200 allele (and thus  also the  pet56 defective) grew much poorer than cells that were wild  type for  PET56 ( his3 - 11,15 allele), we investigated  whether the difference was because of reduced cell viability and/or mtDNA  instability for the  his3delta 200-containing strains.	gene_phenotype
69969	2	334059	7	NULL	NULL	0	NULL	PET56	GP	wild type	shows					growth	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_89	12840009	Because strains carrying the  his3delta 200 allele (and thus  also the  pet56 defective) grew much poorer than cells that were wild  type for  PET56 ( his3 - 11,15 allele), we investigated  whether the difference was because of reduced cell viability and/or mtDNA  instability for the  his3delta 200-containing strains.	gene_phenotype
69970	3	334059	7	NULL	NULL	0	NULL	statement 1	Process		is poorer than					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_89	12840009	Because strains carrying the  his3delta 200 allele (and thus  also the  pet56 defective) grew much poorer than cells that were wild  type for  PET56 ( his3 - 11,15 allele), we investigated  whether the difference was because of reduced cell viability and/or mtDNA  instability for the  his3delta 200-containing strains.	gene_phenotype
69971	4	334059	7	NULL	NULL	NULL	NULL	PET56	GP		contains					his3 - 11,15 allele	Chromosome				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_89	12840009	Because strains carrying the  his3delta 200 allele (and thus  also the  pet56 defective) grew much poorer than cells that were wild  type for  PET56 ( his3 - 11,15 allele), we investigated  whether the difference was because of reduced cell viability and/or mtDNA  instability for the  his3delta 200-containing strains.	gene_phenotype
69974	1	334060	7	NULL	NULL	NULL	NULL	PET56	GP		increase					CRD1	GP	cell viability of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_103	12840009	When YPH500 and YZD2,  carrying the  his3delta 200 allele with its associated  defective  pet56, were supplied with a plasmid-borne copy of   PET56, cell viability for both the  CRD1 and   crd1delta strains was significantly increased particularly when  they were plated on YPEG for which mitochondrial function is required.	gene_phenotype
69975	2	334060	7	NULL	NULL	0	NULL	PET56	GP		increase					crd1delta strains	GP	cell viability of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_103	12840009	When YPH500 and YZD2,  carrying the  his3delta 200 allele with its associated  defective  pet56, were supplied with a plasmid-borne copy of   PET56, cell viability for both the  CRD1 and   crd1delta strains was significantly increased particularly when  they were plated on YPEG for which mitochondrial function is required.	gene_phenotype
69976	1	334061	7	NULL	NULL	0	NULL	crd1delta	GP	mutant	shows					poor growth	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_192	12840009	The poor viability  properties of YPH500 and YZD2 were largely corrected by introducing a  plasmid-borne copy of  PET56 confirming that the synergistic effects  of the  crd1delta and  pet56 mutations were the primary  reason for the poor growth properties rather than the lack of CL.	gene_phenotype
69977	2	334061	7	NULL	NULL	NULL	NULL	pet56 	GP	mutant	shows					poor growth	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_192	12840009	The poor viability  properties of YPH500 and YZD2 were largely corrected by introducing a  plasmid-borne copy of  PET56 confirming that the synergistic effects  of the  crd1delta and  pet56 mutations were the primary  reason for the poor growth properties rather than the lack of CL.	gene_phenotype
69978	3	334061	7	NULL	NULL	0	NULL	CL	Chemical	lack of	does not contribute to					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_192	12840009	The poor viability  properties of YPH500 and YZD2 were largely corrected by introducing a  plasmid-borne copy of  PET56 confirming that the synergistic effects  of the  crd1delta and  pet56 mutations were the primary  reason for the poor growth properties rather than the lack of CL.	gene_phenotype
69979	4	334061	7	NULL	NULL	0	NULL	CL	Chemical	lack of	does not contribute to					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_192	12840009	The poor viability  properties of YPH500 and YZD2 were largely corrected by introducing a  plasmid-borne copy of  PET56 confirming that the synergistic effects  of the  crd1delta and  pet56 mutations were the primary  reason for the poor growth properties rather than the lack of CL.	gene_phenotype
69980	1	334062	7	NULL	NULL	0	NULL	crd1delta	GP	mutant	forms					petite	cell				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_125	15169766	In the  PET56 background as well,  crd1delta mutant cells exhibited a higher frequency of petite formation than did the wild type when grown at 39  degrees C.	gene_phenotype
69981	2	334062	7	NULL	NULL	0	NULL	statement 1	Process		occur at					PET56 background	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_125	15169766	In the  PET56 background as well,  crd1delta mutant cells exhibited a higher frequency of petite formation than did the wild type when grown at 39  degrees C.	gene_phenotype
69985	3	334062	7	NULL	NULL	0	NULL	crd1delta	GP	wild type	forms					petite	Cell				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_125	15169766	In the  PET56 background as well,  crd1delta mutant cells exhibited a higher frequency of petite formation than did the wild type when grown at 39  degrees C.	gene_phenotype
69986	4	334062	7	NULL	NULL	0	NULL	statement 1	Process		higher frequecy than					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_125	15169766	In the  PET56 background as well,  crd1delta mutant cells exhibited a higher frequency of petite formation than did the wild type when grown at 39  degrees C.	gene_phenotype
69987	1	334063	7	NULL	NULL	0	NULL	CRD1	GP	expression of	reduces					petite cells	cell				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_126	15169766	In both strain backgrounds, expression of  CRD1 led to a reduction in the number of petite cells in the  crd1delta mutant to wild type levels, whereas the expression of  PET56 had no effect.	gene_phenotype
69988	2	334063	7	NULL	NULL	0	NULL	statement 1	Process		occur in					crd1delta	GP	mutant			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_126	15169766	In both strain backgrounds, expression of  CRD1 led to a reduction in the number of petite cells in the  crd1delta mutant to wild type levels, whereas the expression of  PET56 had no effect.	gene_phenotype
69989	3	334063	7	NULL	NULL	NULL	NULL	statement 1	Process		is reduced to					crd1delta	GP	wild type			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_126	15169766	In both strain backgrounds, expression of  CRD1 led to a reduction in the number of petite cells in the  crd1delta mutant to wild type levels, whereas the expression of  PET56 had no effect.	gene_phenotype
69990	4	334063	7	NULL	NULL	0	NULL	PET56	GP	expression of	does not effect					petite cells	Cell				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_31_32294_s_126	15169766	In both strain backgrounds, expression of  CRD1 led to a reduction in the number of petite cells in the  crd1delta mutant to wild type levels, whereas the expression of  PET56 had no effect.	gene_phenotype
69991	1	334065	7	NULL	NULL	NULL	NULL	mitochondrial DNA	NucleicAcid	instability of	is due to					PET56 gene	GP	reduced expression of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_7	12840009	We present evidence that  mitochondrial DNA instability, loss of viability, and defects in the ETS  exhibited at elevated temperatures by some mutants are caused by the reduced  expression of the  PET56 gene in the presence of the   his3delta 200 allele and not the lack of CL alone.	gene_phenotype
69992	2	334065	7	NULL	NULL	0	NULL	viability	Process	loss of	is due to					PET56 gene	GP	reduced expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_7	12840009	We present evidence that  mitochondrial DNA instability, loss of viability, and defects in the ETS  exhibited at elevated temperatures by some mutants are caused by the reduced  expression of the  PET56 gene in the presence of the   his3delta 200 allele and not the lack of CL alone.	gene_phenotype
69993	3	334065	7	NULL	NULL	NULL	NULL	ETS	Process	defects in	is due to					PET56 gene	GP	reduced expression of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_7	12840009	We present evidence that  mitochondrial DNA instability, loss of viability, and defects in the ETS  exhibited at elevated temperatures by some mutants are caused by the reduced  expression of the  PET56 gene in the presence of the   his3delta 200 allele and not the lack of CL alone.	gene_phenotype
69995	4	334065	7	NULL	NULL	0	NULL	statement 1	Process		in the presence of					his3delta 200 allele	Chromosome				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_7	12840009	We present evidence that  mitochondrial DNA instability, loss of viability, and defects in the ETS  exhibited at elevated temperatures by some mutants are caused by the reduced  expression of the  PET56 gene in the presence of the   his3delta 200 allele and not the lack of CL alone.	gene_phenotype
69996	5	334065	7	NULL	NULL	0	NULL	statement 2	Process		in the presence of					his3delta 200 allele	Chromosome				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_7	12840009	We present evidence that  mitochondrial DNA instability, loss of viability, and defects in the ETS  exhibited at elevated temperatures by some mutants are caused by the reduced  expression of the  PET56 gene in the presence of the   his3delta 200 allele and not the lack of CL alone.	gene_phenotype
69997	6	334065	7	NULL	NULL	0	NULL	statement 3	Process		in the presence of					his3delta 200 allele	Chromosome				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_7	12840009	We present evidence that  mitochondrial DNA instability, loss of viability, and defects in the ETS  exhibited at elevated temperatures by some mutants are caused by the reduced  expression of the  PET56 gene in the presence of the   his3delta 200 allele and not the lack of CL alone.	gene_phenotype
69998	7	334065	7	NULL	NULL	0	NULL	statement 1	Process		not the lack of					CL	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_7	12840009	We present evidence that  mitochondrial DNA instability, loss of viability, and defects in the ETS  exhibited at elevated temperatures by some mutants are caused by the reduced  expression of the  PET56 gene in the presence of the   his3delta 200 allele and not the lack of CL alone.	gene_phenotype
69999	8	334065	7	NULL	NULL	0	NULL	statement 2	Process		not the lack of					CL	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_7	12840009	We present evidence that  mitochondrial DNA instability, loss of viability, and defects in the ETS  exhibited at elevated temperatures by some mutants are caused by the reduced  expression of the  PET56 gene in the presence of the   his3delta 200 allele and not the lack of CL alone.	gene_phenotype
70000	9	334065	7	NULL	NULL	0	NULL	statement 3	Process		not the lack of					CL	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_7	12840009	We present evidence that  mitochondrial DNA instability, loss of viability, and defects in the ETS  exhibited at elevated temperatures by some mutants are caused by the reduced  expression of the  PET56 gene in the presence of the   his3delta 200 allele and not the lack of CL alone.	gene_phenotype
70001	1	334066	7	NULL	NULL	NULL	NULL	small colonies	Cell		obtained with					mrm2delta strain	Organism	high frequency of			NULL		NULL	NULL	NULL	NULL	gw60_embo_21_5_1139_s_66	11867542	After passing several generations on glucose medium, small colonies were obtained with high frequency for the  mrm2delta strain (Figure  2B), reminiscent of the cytoplasmic petite colonies obtained with a strain disrupted for  PET56 ( Sirum-Connolly and Mason, 1993).	gene_phenotype
70002	2	334066	7	NULL	NULL	0	NULL	statement 1	Process		occur in					glucose medium	Chemical				NULL		0	NULL	NULL	NULL	gw60_embo_21_5_1139_s_66	11867542	After passing several generations on glucose medium, small colonies were obtained with high frequency for the  mrm2delta strain (Figure  2B), reminiscent of the cytoplasmic petite colonies obtained with a strain disrupted for  PET56 ( Sirum-Connolly and Mason, 1993).	gene_phenotype
70003	3	334066	7	NULL	NULL	0	NULL	cytoplasmic petite colonies 	Cell	reminiscent of 	obtained upon					strain disrupted for PET56	Organism				NULL		0	NULL	NULL	NULL	gw60_embo_21_5_1139_s_66	11867542	After passing several generations on glucose medium, small colonies were obtained with high frequency for the  mrm2delta strain (Figure  2B), reminiscent of the cytoplasmic petite colonies obtained with a strain disrupted for  PET56 ( Sirum-Connolly and Mason, 1993).	gene_phenotype
70004	1	334067	7	NULL	NULL	0	NULL	CRD1 cells	Cell		transcription level of		high			PET56	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_98	12840009	There was little statistical difference in viability between   crd1delta and  CRD1 cells with a high transcription level  of  PET56 (YZD5 and DL1, respectively) when grown in YPD and plated on  YPD plates ( Fig. 2,  first  bar in each strain set), whereas  crd1delta cells (YZD2) with a  low transcription level of  PET56 showed a 40% reduction in cell  viability compared with its  CRD1 parental strain (YPH500).	gene_phenotype
70005	2	334067	7	NULL	NULL	0	NULL	crd1delta	GP	viability of	is different from					statement 1	Process	viability of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_98	12840009	There was little statistical difference in viability between   crd1delta and  CRD1 cells with a high transcription level  of  PET56 (YZD5 and DL1, respectively) when grown in YPD and plated on  YPD plates ( Fig. 2,  first  bar in each strain set), whereas  crd1delta cells (YZD2) with a  low transcription level of  PET56 showed a 40% reduction in cell  viability compared with its  CRD1 parental strain (YPH500).	gene_phenotype
70006	3	334067	7	NULL	NULL	0	NULL	crd1delta cells	Cell		transcription level of		low			PET56	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_98	12840009	There was little statistical difference in viability between   crd1delta and  CRD1 cells with a high transcription level  of  PET56 (YZD5 and DL1, respectively) when grown in YPD and plated on  YPD plates ( Fig. 2,  first  bar in each strain set), whereas  crd1delta cells (YZD2) with a  low transcription level of  PET56 showed a 40% reduction in cell  viability compared with its  CRD1 parental strain (YPH500).	gene_phenotype
70007	4	334067	7	NULL	NULL	0	NULL	statement 3	Process	viability of	is less than					statement 1	Process	viability of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35204_s_98	12840009	There was little statistical difference in viability between   crd1delta and  CRD1 cells with a high transcription level  of  PET56 (YZD5 and DL1, respectively) when grown in YPD and plated on  YPD plates ( Fig. 2,  first  bar in each strain set), whereas  crd1delta cells (YZD2) with a  low transcription level of  PET56 showed a 40% reduction in cell  viability compared with its  CRD1 parental strain (YPH500).	gene_phenotype
70008	1	334069	7	NULL	NULL	0	NULL	E.coli cell extracts	Cell		carry					nagK	GP				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_2_700_s_188	11133965	Cell extracts of  E. coli(pWWF52) carrying  nagK inserted in pET5a (Table  1) showed no activity against fumarylpyruvate, formed from gentisate by the joint action of NagI and NagK, even though SDS-PAGE of induced cells showed a polypeptide of the right size (~21 kDa) expressed from this construct (data not shown); we assume that the high levels of expression produced an insoluble product in inclusion bodies.	gene_phenotype
70009	2	334069	7	NULL	NULL	NULL	NULL	statement 1	Process		 no activity against					fumarylpyruvate	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_2_700_s_188	11133965	Cell extracts of  E. coli(pWWF52) carrying  nagK inserted in pET5a (Table  1) showed no activity against fumarylpyruvate, formed from gentisate by the joint action of NagI and NagK, even though SDS-PAGE of induced cells showed a polypeptide of the right size (~21 kDa) expressed from this construct (data not shown); we assume that the high levels of expression produced an insoluble product in inclusion bodies.	gene_phenotype
70010	1	334070	7	NULL	NULL	0	NULL	S. cerevisiae 	Organism		is orthologous to					S. bayanus 	Organism				NULL		0	NULL	NULL	NULL	gw60_genetics_154_3_999_s_177	10757749	Sequence comparisons among specific translational activators from budding yeasts:   Comparison of the proteins coded by orthologous genes of the sister species  S. cerevisiae and  S. bayanus reveals that they are all similar in sequence: 73% identity for Pet111p, 72% for Pet54p and Pet122p, and 76% for Pet494p.	gene_phenotype
70011	2	334070	7	NULL	NULL	0	NULL	S. cerevisiae	Organism	sequence of	is similar to					S. bayanus 	Organism	sequence of			NULL		0	NULL	NULL	NULL	gw60_genetics_154_3_999_s_177	10757749	Sequence comparisons among specific translational activators from budding yeasts:   Comparison of the proteins coded by orthologous genes of the sister species  S. cerevisiae and  S. bayanus reveals that they are all similar in sequence: 73% identity for Pet111p, 72% for Pet54p and Pet122p, and 76% for Pet494p.	gene_phenotype
70012	1	334071	7	NULL	NULL	NULL	NULL	pre- RPR1 complex 	GP		shows					catalytic activity	Process				NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_71_0_165_s_156	12045094	Consistent  with this, recent studies have shown that the pre- RPR1 complex has catalytic activity (C. Srisawat, personal communication), which is not  surprising considering that each of the protein subunits in the mature holoenzyme  can immunoprecipitate the pre- RPR1 RNA.	gene_phenotype
70013	2	334071	7	NULL	NULL	0	NULL	mature holoenzyme	GP		bind			protein subunit		pre- RPR1 RNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_71_0_165_s_156	12045094	Consistent  with this, recent studies have shown that the pre- RPR1 complex has catalytic activity (C. Srisawat, personal communication), which is not  surprising considering that each of the protein subunits in the mature holoenzyme  can immunoprecipitate the pre- RPR1 RNA.	gene_phenotype
70014	1	334074	7	NULL	NULL	0	NULL	RPR1 RNA	NucleicAcid	accumulation of	is defecient in					mutant cells	Cell				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_10_3264_s_196	11971960	The accumulation of RPR1 RNA was also deficient in mutant cells and the proportion of mature to pre-RPR1 RNA was very different (Fig.  5D).	gene_phenotype
70015	1	334075	7	NULL	NULL	0	NULL	 RNase P	GP	nuclear	is a type of					RNA-based enzyme	GP				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_71_0_165_s_218	12045094	The importance of the critical regions in the  yeast  RPR1 RNA for RNase P activity supports the hypothesis that nuclear RNase P is an RNA-based  enzyme.	gene_phenotype
70016	2	334075	7	NULL	NULL	0	NULL	RPR1 RNA	NucleicAcid	critical regions in;;yeast	shows					RNase P activity	Process				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_71_0_165_s_218	12045094	The importance of the critical regions in the  yeast  RPR1 RNA for RNase P activity supports the hypothesis that nuclear RNase P is an RNA-based  enzyme.	gene_phenotype
70017	3	334075	7	NULL	NULL	0	NULL	statement 2	Process		support					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_71_0_165_s_218	12045094	The importance of the critical regions in the  yeast  RPR1 RNA for RNase P activity supports the hypothesis that nuclear RNase P is an RNA-based  enzyme.	gene_phenotype
70018	1	334076	7	NULL	NULL	0	NULL	RNase P	GP	wild-type	localizes to			RNA subunit of		nucleolus	CellComponent				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_16_2463_s_80	9716399	The fluorescent probe to the wild-type RNA subunit of RNase P,  RPR1 RNA, showed clear localization of most of the signal to the nucleolus (Fig.  4a-c).	gene_phenotype
70019	2	334076	7	NULL	NULL	0	NULL	RPR1 RNA	NucleicAcid		localizes to					nucleolus	CellComponent				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_16_2463_s_80	9716399	The fluorescent probe to the wild-type RNA subunit of RNase P,  RPR1 RNA, showed clear localization of most of the signal to the nucleolus (Fig.  4a-c).	gene_phenotype
70020	1	334078	7	NULL	NULL	0	NULL	RNase P	GP	mutation in	leads to			RNA subunit		 5.8 rRNA	NucleicAcid	accumulation of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_12_7897_s_251	10567516	Interestingly, a mutation in the RNase P RNA subunit ( rpr1) leads to the accumulation of an aberrant form of 5.8 rRNA that is 3' extended for about 30 nucleotides ( 28).	gene_phenotype
70021	2	334078	7	NULL	NULL	0	NULL	 5.8 rRNA	NucleicAcid		is extended for					30 nucleotides	Chemical				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_12_7897_s_251	10567516	Interestingly, a mutation in the RNase P RNA subunit ( rpr1) leads to the accumulation of an aberrant form of 5.8 rRNA that is 3' extended for about 30 nucleotides ( 28).	gene_phenotype
70022	3	334078	7	NULL	NULL	0	NULL	RNase P	GP		is			RNA subunit		rpr1	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_12_7897_s_251	10567516	Interestingly, a mutation in the RNase P RNA subunit ( rpr1) leads to the accumulation of an aberrant form of 5.8 rRNA that is 3' extended for about 30 nucleotides ( 28).	gene_phenotype
70023	1	334079	7	NULL	NULL	0	NULL	RNase P	GP	yeast;;nuclear	important role in			P4		pre-tRNA	NucleicAcid	binding of			NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_71_0_165_s_180	12045094	For yeast nuclear  RNase P, mutagenesis studies of the conserved nucleotides within and near P4 have  suggested an important role in pre-tRNA binding, catalysis, and  RPR1 RNA maturation ( 103).	gene_phenotype
70024	2	334079	7	NULL	NULL	0	NULL	RNase P	GP	yeast;;nuclear	important role in			P4		catalysis	Process				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_71_0_165_s_180	12045094	For yeast nuclear  RNase P, mutagenesis studies of the conserved nucleotides within and near P4 have  suggested an important role in pre-tRNA binding, catalysis, and  RPR1 RNA maturation ( 103).	gene_phenotype
70025	3	334079	7	NULL	NULL	0	NULL	RNase P	GP	yeast;;nuclear	important role in			P4		RPR1 RNA	NucleicAcid	maturation of			NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_71_0_165_s_180	12045094	For yeast nuclear  RNase P, mutagenesis studies of the conserved nucleotides within and near P4 have  suggested an important role in pre-tRNA binding, catalysis, and  RPR1 RNA maturation ( 103).	gene_phenotype
70026	1	334080	7	NULL	NULL	0	NULL	tRNA methyltransferase 	GP	activity of	contributes to					RPR1 RNA	NucleicAcid	stability of			NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_71_0_165_s_256	12045094	Previous work has  linked a tRNA methyltransferase activity to the stability of  RPR1 RNA ( 136), although none of the identified subunits have any detectable sequence homology  to known tRNA processing or modification enzymes.	gene_phenotype
70027	1	334083	7	NULL	NULL	0	NULL	RNase P	GP	yeast	composed of					RPR1 RNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_10_3264_s_285	11971960	Yeast RNase P is also composed of one RNA subunit (RPR1 RNA) and nine protein subunits that are all essential for cell viability ( 8,  11,  16,  38,  41,  59).	gene_phenotype
70028	2	334083	7	NULL	NULL	NULL	NULL	RNA subunit	NucleicAcid		is a type of					RPR1 RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_10_3264_s_285	11971960	Yeast RNase P is also composed of one RNA subunit (RPR1 RNA) and nine protein subunits that are all essential for cell viability ( 8,  11,  16,  38,  41,  59).	gene_phenotype
70029	3	334083	7	NULL	NULL	0	NULL	RNase P	GP	yeast	composed of					protein subunits	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_10_3264_s_285	11971960	Yeast RNase P is also composed of one RNA subunit (RPR1 RNA) and nine protein subunits that are all essential for cell viability ( 8,  11,  16,  38,  41,  59).	gene_phenotype
70030	4	334083	7	NULL	NULL	0	NULL	statement 3	GP		is essential for					cell viability	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_10_3264_s_285	11971960	Yeast RNase P is also composed of one RNA subunit (RPR1 RNA) and nine protein subunits that are all essential for cell viability ( 8,  11,  16,  38,  41,  59).	gene_phenotype
70204	1	334085	7	NULL	NULL	NULL	NULL	hcPUS4	GP	presence of	leads to					tRNA precursor	NucleicAcid	accumulation of			NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_mol-cell-biol_20_7_10713174_s_6	10713174	The presence of hcPUS4 or hcNME1 led to the accumulation of certain  tRNA precursors, and their Gcd(-) phenotypes were reversed by overexpressing  the RNA component of RNase P (RPR1), responsible for 5''-end processing  of all tRNAs.	gene_phenotype
70205	2	334085	7	NULL	NULL	0	NULL	hcNME1	GP	presence of	leads to					tRNA precursor	NucleicAcid	accumulation of			NULL		0	NULL	NULL	NULL	abs-batch0517-0529_mol-cell-biol_20_7_10713174_s_6	10713174	The presence of hcPUS4 or hcNME1 led to the accumulation of certain  tRNA precursors, and their Gcd(-) phenotypes were reversed by overexpressing  the RNA component of RNase P (RPR1), responsible for 5''-end processing  of all tRNAs.	gene_phenotype
70206	3	334085	7	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_mol-cell-biol_20_7_10713174_s_6	10713174	The presence of hcPUS4 or hcNME1 led to the accumulation of certain  tRNA precursors, and their Gcd(-) phenotypes were reversed by overexpressing  the RNA component of RNase P (RPR1), responsible for 5''-end processing  of all tRNAs.	gene_phenotype
70207	4	334085	7	NULL	NULL	NULL	NULL	Gcd(-) phenotype	Process		reversed by					RNase P	GP	overexpressing	RNA component of		NULL		NULL	NULL	NULL	NULL	abs-batch0517-0529_mol-cell-biol_20_7_10713174_s_6	10713174	The presence of hcPUS4 or hcNME1 led to the accumulation of certain  tRNA precursors, and their Gcd(-) phenotypes were reversed by overexpressing  the RNA component of RNase P (RPR1), responsible for 5''-end processing  of all tRNAs.	gene_phenotype
70208	5	334085	7	NULL	NULL	0	NULL	RNase P	GP		is			RNA component		RPR1	NucleicAcid				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_mol-cell-biol_20_7_10713174_s_6	10713174	The presence of hcPUS4 or hcNME1 led to the accumulation of certain  tRNA precursors, and their Gcd(-) phenotypes were reversed by overexpressing  the RNA component of RNase P (RPR1), responsible for 5''-end processing  of all tRNAs.	gene_phenotype
70209	6	334085	7	NULL	NULL	0	NULL	RNase P	GP		responsible for					tRNA	NucleicAcid			 5''-end processing of	NULL		0	NULL	NULL	NULL	abs-batch0517-0529_mol-cell-biol_20_7_10713174_s_6	10713174	The presence of hcPUS4 or hcNME1 led to the accumulation of certain  tRNA precursors, and their Gcd(-) phenotypes were reversed by overexpressing  the RNA component of RNase P (RPR1), responsible for 5''-end processing  of all tRNAs.	gene_phenotype
70210	1	334089	7	NULL	NULL	0	NULL	Lsm2 - Lsm7 complex 	GP		is not required for					snR5 RNA	NucleicAcid	accumulation of			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_6_2842_s_288	15075370	Thus, the Lsm2 - Lsm7 complex does not appear to be required for the accumulation of snR5 RNA or for its role in pseudouridylation.	gene_phenotype
70211	2	334089	7	NULL	NULL	0	NULL	Lsm2 - Lsm7 complex	GP		is not required for					pseudouridylation	Process	role in			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_6_2842_s_288	15075370	Thus, the Lsm2 - Lsm7 complex does not appear to be required for the accumulation of snR5 RNA or for its role in pseudouridylation.	gene_phenotype
70212	1	334090	7	NULL	NULL	NULL	NULL	elements	NucleicAcid		essential for					RNA	NucleicAcid	accumulation of			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_2_457_s_48	9889201	Since the actin mRNA was expressed correctly (data not shown), we concluded that the snR5 RNA lacks elements that are essential for RNA accumulation.	gene_phenotype
70217	2	334090	7	NULL	NULL	0	NULL	snR5 RNA	NucleicAcid		lacks					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_2_457_s_48	9889201	Since the actin mRNA was expressed correctly (data not shown), we concluded that the snR5 RNA lacks elements that are essential for RNA accumulation.	gene_phenotype
70220	1	334091	7	NULL	NULL	0	NULL	Lsm Proteins	GP		is not required for					snR5 RNA	NucleicAcid	accumulation of			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_6_2842_s_246	15075370	Lsm Proteins Are Not Required for snR5 RNA Accumulation or Its Function in Pseudouridylation   To examine the role of Lsm proteins in snR5 function, we used strains in which  LSM2, LSM3, and  LSM8 were under control of the glucose-repressible  GAL promoter (Mayes  et al., 1999 ) to deplete the proteins.	gene_phenotype
70221	2	334091	7	NULL	NULL	0	NULL	Lsm Proteins	GP		is not required for					Pseudouridylation	Process	function in			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_6_2842_s_246	15075370	Lsm Proteins Are Not Required for snR5 RNA Accumulation or Its Function in Pseudouridylation   To examine the role of Lsm proteins in snR5 function, we used strains in which  LSM2, LSM3, and  LSM8 were under control of the glucose-repressible  GAL promoter (Mayes  et al., 1999 ) to deplete the proteins.	gene_phenotype
70222	3	334091	7	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_6_2842_s_246	15075370	Lsm Proteins Are Not Required for snR5 RNA Accumulation or Its Function in Pseudouridylation   To examine the role of Lsm proteins in snR5 function, we used strains in which  LSM2, LSM3, and  LSM8 were under control of the glucose-repressible  GAL promoter (Mayes  et al., 1999 ) to deplete the proteins.	gene_phenotype
70223	1	334092	7	NULL	NULL	0	NULL	SNR5	NucleicAcid		supports				promoter	transcription	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_2_457_s_71	9889201	The differences in the levels of RNA accumulation probably reflect the fact that the  SNR5 promoter supports transcription more efficiently than does the  ADH promoter.	gene_phenotype
70224	2	334092	7	NULL	NULL	0	NULL	ADH	GP		supports				promoter	transcription	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_2_457_s_71	9889201	The differences in the levels of RNA accumulation probably reflect the fact that the  SNR5 promoter supports transcription more efficiently than does the  ADH promoter.	gene_phenotype
70225	3	334092	7	NULL	NULL	0	NULL	statement 1	Process		is more efficient than					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_2_457_s_71	9889201	The differences in the levels of RNA accumulation probably reflect the fact that the  SNR5 promoter supports transcription more efficiently than does the  ADH promoter.	gene_phenotype
70226	1	334093	7	NULL	NULL	NULL	NULL	U1003 residue	Chemical		converted to		site-specifically			pseudouridine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_89_5_799_s_190	9182768	Mapping the pseudouridylation sites in 25S rRNA isolated from the deltasnR5/RES strain  demonstrated that restoration of the accumulation of snR5 RNA reestablished the site-specific  conversion of U1003 and U1123 residues into pseudouridine (  Figure 6, lanes 3 and 6).	gene_phenotype
70227	2	334093	7	NULL	NULL	NULL	NULL	U1123 residue	Chemical		converted to		site-specifically			pseudouridine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cell_89_5_799_s_190	9182768	Mapping the pseudouridylation sites in 25S rRNA isolated from the deltasnR5/RES strain  demonstrated that restoration of the accumulation of snR5 RNA reestablished the site-specific  conversion of U1003 and U1123 residues into pseudouridine (  Figure 6, lanes 3 and 6).	gene_phenotype
70228	3	334093	7	NULL	NULL	NULL	NULL	snR5 RNA	NucleicAcid		reestablishes					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_89_5_799_s_190	9182768	Mapping the pseudouridylation sites in 25S rRNA isolated from the deltasnR5/RES strain  demonstrated that restoration of the accumulation of snR5 RNA reestablished the site-specific  conversion of U1003 and U1123 residues into pseudouridine (  Figure 6, lanes 3 and 6).	gene_phenotype
70229	4	334093	7	NULL	NULL	NULL	NULL	snR5 RNA	NucleicAcid		reestablishes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_cell_89_5_799_s_190	9182768	Mapping the pseudouridylation sites in 25S rRNA isolated from the deltasnR5/RES strain  demonstrated that restoration of the accumulation of snR5 RNA reestablished the site-specific  conversion of U1003 and U1123 residues into pseudouridine (  Figure 6, lanes 3 and 6).	gene_phenotype
70231	1	334094	7	NULL	NULL	0	NULL	RPL7A	GP		harbors					snR39	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_8_2981_s_336	15798187	Deletion of RPL7A that harbors snR39 within its introns moderately impairs growth and affects budding ( ); however, deletion of RPL7B that harbors snR59 in its intron has no effect on growth ( ).	gene_phenotype
70232	2	334094	7	NULL	NULL	0	NULL	 RPL7A	GP	deletion of	impairs		moderately			growth	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_8_2981_s_336	15798187	Deletion of RPL7A that harbors snR39 within its introns moderately impairs growth and affects budding ( ); however, deletion of RPL7B that harbors snR59 in its intron has no effect on growth ( ).	gene_phenotype
70233	3	334094	7	NULL	NULL	NULL	NULL	 RPL7A	GP	deletion of	affects		moderately			budding	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_2981_s_336	15798187	Deletion of RPL7A that harbors snR39 within its introns moderately impairs growth and affects budding ( ); however, deletion of RPL7B that harbors snR59 in its intron has no effect on growth ( ).	gene_phenotype
70234	4	334094	7	NULL	NULL	0	NULL	RPL7B	GP		harbors					snR59	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_8_2981_s_336	15798187	Deletion of RPL7A that harbors snR39 within its introns moderately impairs growth and affects budding ( ); however, deletion of RPL7B that harbors snR59 in its intron has no effect on growth ( ).	gene_phenotype
70235	5	334094	7	NULL	NULL	NULL	NULL	RPL7B	Process	deletion of	has no effect on					growth	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_8_2981_s_336	15798187	Deletion of RPL7A that harbors snR39 within its introns moderately impairs growth and affects budding ( ); however, deletion of RPL7B that harbors snR59 in its intron has no effect on growth ( ).	gene_phenotype
70236	1	334095	7	NULL	NULL	0	NULL	U65/U24 transcript	NucleicAcid		carries					U65 sequence	GP	mutant			NULL		0	NULL	NULL	NULL	gw60_embo_18_2_457_s_128	9889201	Therefore, a U65/U24 fusion snoRNA was constructed and placed under the control of the  SNR5 promoter (Figure  4A), anticipating that the U65/U24 transcript, even if carrying mutant U65 sequences, would be stable in yeast cells due to the presence of the 5''-terminal cap structure and the 3''-terminal U24 snoRNP particle.	gene_phenotype
70237	2	334095	7	NULL	NULL	0	NULL	statement 1	Process		stable in					yeast cells	Cell				NULL		0	NULL	NULL	NULL	gw60_embo_18_2_457_s_128	9889201	Therefore, a U65/U24 fusion snoRNA was constructed and placed under the control of the  SNR5 promoter (Figure  4A), anticipating that the U65/U24 transcript, even if carrying mutant U65 sequences, would be stable in yeast cells due to the presence of the 5''-terminal cap structure and the 3''-terminal U24 snoRNP particle.	gene_phenotype
70238	3	334095	7	NULL	NULL	NULL	NULL	statement 2	Process		due to					 cap structure	Process	presence of		5''-terminal	NULL		NULL	NULL	NULL	NULL	gw60_embo_18_2_457_s_128	9889201	Therefore, a U65/U24 fusion snoRNA was constructed and placed under the control of the  SNR5 promoter (Figure  4A), anticipating that the U65/U24 transcript, even if carrying mutant U65 sequences, would be stable in yeast cells due to the presence of the 5''-terminal cap structure and the 3''-terminal U24 snoRNP particle.	gene_phenotype
70239	4	334095	7	NULL	NULL	NULL	NULL	statement 2	Process		due to					U24 snoRNP particle	NucleicAcid	presence of		3''-terminal	NULL		NULL	NULL	NULL	NULL	gw60_embo_18_2_457_s_128	9889201	Therefore, a U65/U24 fusion snoRNA was constructed and placed under the control of the  SNR5 promoter (Figure  4A), anticipating that the U65/U24 transcript, even if carrying mutant U65 sequences, would be stable in yeast cells due to the presence of the 5''-terminal cap structure and the 3''-terminal U24 snoRNP particle.	gene_phenotype
70240	1	334096	7	NULL	NULL	NULL	NULL			mutation in	cause				repeat 1	snR13F RNA	NucleicAcid	decreased accumulation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6885_s_401	9819377	The mutation in repeat 1 caused decreased accumulation of snR13F RNA without a concomitant increase in 5''-truncated snR13T and 3''-extended snR13RR.	gene_phenotype
70241	2	334096	7	NULL	NULL	NULL	NULL	statement 1	Process		does not increase					snR13T	NucleicAcid			5''-truncated	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6885_s_401	9819377	The mutation in repeat 1 caused decreased accumulation of snR13F RNA without a concomitant increase in 5''-truncated snR13T and 3''-extended snR13RR.	gene_phenotype
70242	3	334096	7	NULL	NULL	0	NULL	statement 1	Process		does not increase					snR13RR	NucleicAcid			3''-extended	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_12_6885_s_401	9819377	The mutation in repeat 1 caused decreased accumulation of snR13F RNA without a concomitant increase in 5''-truncated snR13T and 3''-extended snR13RR.	gene_phenotype
70243	1	334097	7	NULL	NULL	NULL	NULL			mutation in	failed to cause				repeat 3	snR13T RNA	NucleicAcid	increase in accumulation			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6885_s_402	9819377	Both of the mutations in repeat 3 failed to cause detectable increases in the accumulation of snR13T and snR13R RNAs.	gene_phenotype
70244	2	334097	7	NULL	NULL	NULL	NULL			mutations in	failed to cause				repeat 3	snR13R RNA	NucleicAcid	increase in accumulation			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6885_s_402	9819377	Both of the mutations in repeat 3 failed to cause detectable increases in the accumulation of snR13T and snR13R RNAs.	gene_phenotype
70245	1	334099	7	NULL	NULL	0	NULL	 Sen1p	GP	inactivation of	accumulate					snR13 RNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_12_6885_s_169	9819377	Kinetics of accumulation of snR13 RNAs following inactivation of Sen1p.	gene_phenotype
70246	1	334102	7	NULL	NULL	0	NULL	snR13F RNA	NucleicAcid		is not essential for					growth	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_12_6885_s_178	9819377	This strain was found to be viable and failed to produce any detectable snR13F RNA as judged by Northern blotting, indicating that the RNA is not essential for growth.	gene_phenotype
70247	1	334103	7	NULL	NULL	0	NULL	nrd1	GP	mutant allele of	reduce					snR13 	NucleicAcid	accumulation of mature			NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_32_8_2441_s_290	15121901	Mutant alleles of  nrd1 and  sen1 exhibit reduced accumulation of mature snR13 and increased accumulation of RNAs that extend through the snR13 transcription termination site and extend to the site of transcription termination of the next downstream gene on the chromosome ( 7, 8, 16).	gene_phenotype
70248	2	334103	7	NULL	NULL	0	NULL	sen1	GP	mutant allele of	reduce					snR13	NucleicAcid	accumulation of mature			NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_32_8_2441_s_290	15121901	Mutant alleles of  nrd1 and  sen1 exhibit reduced accumulation of mature snR13 and increased accumulation of RNAs that extend through the snR13 transcription termination site and extend to the site of transcription termination of the next downstream gene on the chromosome ( 7, 8, 16).	gene_phenotype
70249	3	334103	7	NULL	NULL	0	NULL	RNAs	NucleicAcid		extend through					snR13	NucleicAcid			transcription termination site	NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_32_8_2441_s_290	15121901	Mutant alleles of  nrd1 and  sen1 exhibit reduced accumulation of mature snR13 and increased accumulation of RNAs that extend through the snR13 transcription termination site and extend to the site of transcription termination of the next downstream gene on the chromosome ( 7, 8, 16).	gene_phenotype
70250	4	334103	7	NULL	NULL	NULL	NULL	RNAs	NucleicAcid		extend to					transcription	Process			 termination site of	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_32_8_2441_s_290	15121901	Mutant alleles of  nrd1 and  sen1 exhibit reduced accumulation of mature snR13 and increased accumulation of RNAs that extend through the snR13 transcription termination site and extend to the site of transcription termination of the next downstream gene on the chromosome ( 7, 8, 16).	gene_phenotype
70251	5	334103	7	NULL	NULL	0	NULL	transcription 	Process		present on				termination site	chromosome	Chromosome			next downstream gene 	NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_32_8_2441_s_290	15121901	Mutant alleles of  nrd1 and  sen1 exhibit reduced accumulation of mature snR13 and increased accumulation of RNAs that extend through the snR13 transcription termination site and extend to the site of transcription termination of the next downstream gene on the chromosome ( 7, 8, 16).	gene_phenotype
70252	6	334103	7	NULL	NULL	0	NULL	statement 3	Process		occur along with					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_32_8_2441_s_290	15121901	Mutant alleles of  nrd1 and  sen1 exhibit reduced accumulation of mature snR13 and increased accumulation of RNAs that extend through the snR13 transcription termination site and extend to the site of transcription termination of the next downstream gene on the chromosome ( 7, 8, 16).	gene_phenotype
70253	7	334103	7	NULL	NULL	0	NULL	nrd1 	GP	mutant allele of	increase					statement 6	Process				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_32_8_2441_s_290	15121901	Mutant alleles of  nrd1 and  sen1 exhibit reduced accumulation of mature snR13 and increased accumulation of RNAs that extend through the snR13 transcription termination site and extend to the site of transcription termination of the next downstream gene on the chromosome ( 7, 8, 16).	gene_phenotype
70254	8	334103	7	NULL	NULL	0	NULL	sen1	GP	mutant allele of	increase					statement 6	Process				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_32_8_2441_s_290	15121901	Mutant alleles of  nrd1 and  sen1 exhibit reduced accumulation of mature snR13 and increased accumulation of RNAs that extend through the snR13 transcription termination site and extend to the site of transcription termination of the next downstream gene on the chromosome ( 7, 8, 16).	gene_phenotype
70255	1	334104	7	NULL	NULL	0	NULL	snR13 transcripts	GP	wild-type	shows					new RNA	NucleicAcid	accumulation in the mutant strain of 			NULL		0	NULL	NULL	NULL	gw60_nature_413_6853_327_s_28	11565036	Northern blot analysis of snR13 and Trs31 transcripts from wild-type and  nrd1 mutant strains shows the accumulation in the mutant strain of a new RNA species, which is larger than the normal Trs31 mRNA, that is detected by probes complementary to either mature snR13 RNA or Trs31 mRNA ( Fig. 1b).	gene_phenotype
70256	2	334104	7	NULL	NULL	0	NULL	Trs31 transcript	GP	wild-type	shows					new RNA	NucleicAcid	accumulation in the mutant strain of 			NULL		0	NULL	NULL	NULL	gw60_nature_413_6853_327_s_28	11565036	Northern blot analysis of snR13 and Trs31 transcripts from wild-type and  nrd1 mutant strains shows the accumulation in the mutant strain of a new RNA species, which is larger than the normal Trs31 mRNA, that is detected by probes complementary to either mature snR13 RNA or Trs31 mRNA ( Fig. 1b).	gene_phenotype
70257	3	334104	7	NULL	NULL	0	NULL	new RNA	NucleicAcid		is larger than					Trs31 mRNA	NucleicAcid	normal			NULL		0	NULL	NULL	NULL	gw60_nature_413_6853_327_s_28	11565036	Northern blot analysis of snR13 and Trs31 transcripts from wild-type and  nrd1 mutant strains shows the accumulation in the mutant strain of a new RNA species, which is larger than the normal Trs31 mRNA, that is detected by probes complementary to either mature snR13 RNA or Trs31 mRNA ( Fig. 1b).	gene_phenotype
70258	1	334105	7	NULL	NULL	0	NULL	 swd2- 3	GP	mutant;;viability of	occur upon					Ref2	GP	overexpression of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_7_2932_s_333	15024081	The viability of the  swd2- 3 and  swd2- 5 mutants at 37 degrees C when Ref2 is overexpressed, together with the recovery of  SNR13 termination, is consistent with this interpretation.	gene_phenotype
70259	2	334105	7	NULL	NULL	0	NULL	swd2- 5	GP	mutant;;viability of	occur upon					Ref2	GP	overexpression of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_7_2932_s_333	15024081	The viability of the  swd2- 3 and  swd2- 5 mutants at 37 degrees C when Ref2 is overexpressed, together with the recovery of  SNR13 termination, is consistent with this interpretation.	gene_phenotype
70260	1	334107	7	NULL	NULL	0	NULL	 snR13	NucleicAcid		is dispensable for					viability	Process				NULL		0	NULL	NULL	NULL	gw60_nature_413_6853_327_s_94	11565036	This function may be more vital to the cell than Nrd1-dependent 3''-end maturation of snoRNAs because most snoRNAs, including snR13, are dispensable for viability.	gene_phenotype
70261	2	334107	7	NULL	NULL	0	NULL	 snR13	NucleicAcid		is a type of					snoRNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_nature_413_6853_327_s_94	11565036	This function may be more vital to the cell than Nrd1-dependent 3''-end maturation of snoRNAs because most snoRNAs, including snR13, are dispensable for viability.	gene_phenotype
70262	3	334107	7	NULL	NULL	0	NULL	snoRNAs	NucleicAcid	maturation of	depends on					Nrd1	GP				NULL		0	NULL	NULL	NULL	gw60_nature_413_6853_327_s_94	11565036	This function may be more vital to the cell than Nrd1-dependent 3''-end maturation of snoRNAs because most snoRNAs, including snR13, are dispensable for viability.	gene_phenotype
70263	1	334108	7	NULL	NULL	0	NULL			mutant	cause				5' C2U4 repeat	snR13F	NucleicAcid	underaccumulation of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_12_6885_s_11	9819377	A mutation in the 5' C2U4 repeat causes underaccumulation of snR13F, whereas mutations in the 3' C2U4 repeat cause the accumulation of two novel RNAs that migrate in the 500-nt range.	gene_phenotype
70264	2	334108	7	NULL	NULL	0	NULL			mutant	cause				 3' C2U4 repeat	snR13F	NucleicAcid	underaccumulation of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_12_6885_s_11	9819377	A mutation in the 5' C2U4 repeat causes underaccumulation of snR13F, whereas mutations in the 3' C2U4 repeat cause the accumulation of two novel RNAs that migrate in the 500-nt range.	gene_phenotype
70265	1	334109	7	NULL	NULL	0	NULL	snR13-RNEW 	NucleicAcid		failed to cause					snR13 RNA	NucleicAcid	accumulation of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_12_6885_s_325	9819377	snR13-RNEW failed to cause any changes in snR13 RNA accumulation (Fig.  9B, lane 5), showing that C2U4 is insufficient by itself to specify a site for 3' end formation in the absence of a proper context.	gene_phenotype
70266	2	334109	7	NULL	NULL	0	NULL				is insufficient 				C2U4	formation	Process	to specify site for		3' end	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_12_6885_s_325	9819377	snR13-RNEW failed to cause any changes in snR13 RNA accumulation (Fig.  9B, lane 5), showing that C2U4 is insufficient by itself to specify a site for 3' end formation in the absence of a proper context.	gene_phenotype
70267	1	334110	7	NULL	NULL	NULL	NULL	snR13 RNA	NucleicAcid	changes in;;accumulation of	result from					Sen1p	GP	requirement of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6885_s_385	9819377	The changes in synthetic rates and levels of accumulation of the snR13 RNAs result from a requirement of Sen1p to both stabilize the 5' terminus and to promote formation of the 3' terminus from a 3''-extended RNA.	gene_phenotype
70268	2	334110	7	NULL	NULL	0	NULL	statement 1	Process		stabilize									5' terminus	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_12_6885_s_385	9819377	The changes in synthetic rates and levels of accumulation of the snR13 RNAs result from a requirement of Sen1p to both stabilize the 5' terminus and to promote formation of the 3' terminus from a 3''-extended RNA.	gene_phenotype
70269	3	334110	7	NULL	NULL	0	NULL				formed from				3' terminus 	3''-extended RNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_12_6885_s_385	9819377	The changes in synthetic rates and levels of accumulation of the snR13 RNAs result from a requirement of Sen1p to both stabilize the 5' terminus and to promote formation of the 3' terminus from a 3''-extended RNA.	gene_phenotype
70270	4	334110	7	NULL	NULL	0	NULL	statement 1	Process		promote					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_12_6885_s_385	9819377	The changes in synthetic rates and levels of accumulation of the snR13 RNAs result from a requirement of Sen1p to both stabilize the 5' terminus and to promote formation of the 3' terminus from a 3''-extended RNA.	gene_phenotype
70271	1	334111	7	NULL	NULL	0	NULL	altered RNA	NucleicAcid	accumulation of	precedes					cell viability	Process	loss of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_12_6885_s_156	9819377	This probe detects [[ only snR13R RNA.                    Because ]]  SEN1 is an essential gene ( 10), we assessed whether the onset of altered RNA accumulation precedes loss of cell viability following a shift to the restrictive temperature.	gene_phenotype
70272	2	334111	7	NULL	NULL	0	NULL	statement 1	Process		followed by					 restrictive temperature		shift to			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_12_6885_s_156	9819377	This probe detects [[ only snR13R RNA.                    Because ]]  SEN1 is an essential gene ( 10), we assessed whether the onset of altered RNA accumulation precedes loss of cell viability following a shift to the restrictive temperature.	gene_phenotype
70273	1	334113	7	NULL	NULL	NULL	NULL	CF IA 	GP		is involved in					chromosomal snoRNA transcripts	NucleicAcid			3"`-end formation of	NULL	rna15- 2 strain	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_5_1379_s_266	11839805	Analysis of the endogenous transcripts produced in a  rna15- 2 strain at the nonpermissive temperature showed the accumulation of a read-through RNA extending inside the gene downstream to the snR13 coding region, showing that CF IA is indeed involved in the 3"`-end formation of chromosomal snoRNA transcripts.	gene_phenotype
70274	1	334114	7	NULL	NULL	NULL	NULL	sen1-1	GP	double mutant	accumulation of		reduce			novel RNAs	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6885_s_12	9819377	At the restrictive temperature, double mutants carrying  sen1-1 and mutations in the 3' C2U4 repeat show reduced accumulation of the novel RNAs and increased accumulation of snR13R RNA, indicating that Sen1p and the 3' C2U4 sequence act in a common pathway to facilitate 3' end formation.	gene_phenotype
70275	2	334114	7	NULL	NULL	NULL	NULL			mutations in	accumulation of		reduce		3' C2U4 repeat 	novel RNAs	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6885_s_12	9819377	At the restrictive temperature, double mutants carrying  sen1-1 and mutations in the 3' C2U4 repeat show reduced accumulation of the novel RNAs and increased accumulation of snR13R RNA, indicating that Sen1p and the 3' C2U4 sequence act in a common pathway to facilitate 3' end formation.	gene_phenotype
70276	3	334114	7	NULL	NULL	0	NULL	sen1-1	GP	double mutant	increase					snR13R RNA	NucleicAcid	accumulation of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_12_6885_s_12	9819377	At the restrictive temperature, double mutants carrying  sen1-1 and mutations in the 3' C2U4 repeat show reduced accumulation of the novel RNAs and increased accumulation of snR13R RNA, indicating that Sen1p and the 3' C2U4 sequence act in a common pathway to facilitate 3' end formation.	gene_phenotype
70277	4	334114	7	NULL	NULL	NULL	NULL			mutations in	increase				 3' C2U4 repeat 	snR13R RNA	NucleicAcid	accumulation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6885_s_12	9819377	At the restrictive temperature, double mutants carrying  sen1-1 and mutations in the 3' C2U4 repeat show reduced accumulation of the novel RNAs and increased accumulation of snR13R RNA, indicating that Sen1p and the 3' C2U4 sequence act in a common pathway to facilitate 3' end formation.	gene_phenotype
70278	5	334114	7	NULL	NULL	NULL	NULL	Sen1p	GP		facilitate					RNA	NucleicAcid			3' end formation 	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6885_s_12	9819377	At the restrictive temperature, double mutants carrying  sen1-1 and mutations in the 3' C2U4 repeat show reduced accumulation of the novel RNAs and increased accumulation of snR13R RNA, indicating that Sen1p and the 3' C2U4 sequence act in a common pathway to facilitate 3' end formation.	gene_phenotype
70279	6	334114	7	NULL	NULL	NULL	NULL				facilitate				 3' C2U4 sequence	RNA	NucleicAcid			 3' end formation	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_12_6885_s_12	9819377	At the restrictive temperature, double mutants carrying  sen1-1 and mutations in the 3' C2U4 repeat show reduced accumulation of the novel RNAs and increased accumulation of snR13R RNA, indicating that Sen1p and the 3' C2U4 sequence act in a common pathway to facilitate 3' end formation.	gene_phenotype
70280	1	334116	7	NULL	NULL	0	NULL	polalphats13 cdc22	GP	Double mutant 	arrested with					cdc22-like phenotype	Process				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_9_8_2107_s_216	9693370	Double mutant  polalphats13 cdc22 ( cdc22 encodes the large subunit of ribonucleotide reductase) arrested with a  cdc22-like phenotype with a very low percent of abnormal nuclear morphology.	gene_phenotype
70281	2	334116	7	NULL	NULL	0	NULL	cdc22	GP		encode					ribonucleotide reductase	GP		large subunit of		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_9_8_2107_s_216	9693370	Double mutant  polalphats13 cdc22 ( cdc22 encodes the large subunit of ribonucleotide reductase) arrested with a  cdc22-like phenotype with a very low percent of abnormal nuclear morphology.	gene_phenotype
70283	1	334118	7	NULL	NULL	0	NULL	cdc22+	GP	overexpression of	did not complement					sporulation deficiency	Process				NULL	cdt2-M1 cells	0	NULL	NULL	NULL	gw70_genetics_164_3_881_s_295	12871901	We found that overexpression of  cdc22+ did not complement the sporulation deficiency of  cdt2-M1 cells (data not shown).	gene_phenotype
70284	1	334119	7	NULL	NULL	0	NULL	checkpoint signal	Process		activates					Cds1p	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_102_16_5797_s_159	15805194	The checkpoint signal that activates Cds1p is generated in the  cdc22 or HU treated cells but not in  orp1 cdc18 cells during the mitotic cell cycle ( ).	gene_phenotype
70285	2	334119	7	NULL	NULL	0	NULL	statement 1	Process		is generated in					cdc22 cells	Cell				NULL		0	NULL	NULL	NULL	gw70_pnas_102_16_5797_s_159	15805194	The checkpoint signal that activates Cds1p is generated in the  cdc22 or HU treated cells but not in  orp1 cdc18 cells during the mitotic cell cycle ( ).	gene_phenotype
70286	3	334119	7	NULL	NULL	0	NULL	statement 1	Process		is generated in					HU treated cells	Cell				NULL		0	NULL	NULL	NULL	gw70_pnas_102_16_5797_s_159	15805194	The checkpoint signal that activates Cds1p is generated in the  cdc22 or HU treated cells but not in  orp1 cdc18 cells during the mitotic cell cycle ( ).	gene_phenotype
70287	4	334119	7	NULL	NULL	0	NULL	statement 1	Process		is not generated in					orp1 cdc18 cells 	Cell				NULL		0	NULL	NULL	NULL	gw70_pnas_102_16_5797_s_159	15805194	The checkpoint signal that activates Cds1p is generated in the  cdc22 or HU treated cells but not in  orp1 cdc18 cells during the mitotic cell cycle ( ).	gene_phenotype
70288	5	334119	7	NULL	NULL	0	NULL	statement 2	Process		occur during					mitotic cell cycle	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_102_16_5797_s_159	15805194	The checkpoint signal that activates Cds1p is generated in the  cdc22 or HU treated cells but not in  orp1 cdc18 cells during the mitotic cell cycle ( ).	gene_phenotype
70289	6	334119	7	NULL	NULL	0	NULL	statement 3	Process		occur during					mitotic cell cycle	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_102_16_5797_s_159	15805194	The checkpoint signal that activates Cds1p is generated in the  cdc22 or HU treated cells but not in  orp1 cdc18 cells during the mitotic cell cycle ( ).	gene_phenotype
70290	7	334119	7	NULL	NULL	0	NULL	statement 4	Process		occur during					mitotic cell cycle	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_102_16_5797_s_159	15805194	The checkpoint signal that activates Cds1p is generated in the  cdc22 or HU treated cells but not in  orp1 cdc18 cells during the mitotic cell cycle ( ).	gene_phenotype
70526	1	334123	7	NULL	NULL	NULL	NULL	rad1- 1 cdc22- M45	Cell	mutant	proceed through					cell division	Process				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_14_3030_s_160	11452028	Some of the quantitative effects reflect the smaller average size of the  rad1- 1 cdc22- M45 mutant cells that proceed through cell division.	gene_phenotype
70643	1	334126	7	NULL	NULL	0	NULL	Spd1p	GP		inhibit					Suc22p activity	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_3_1778_s_90	16317005	To differentiate between inhibition of Suc22p and Cdc22p activity by Spd1p, we took advantage of the observation that budding yeast Rnr1p forms an active RNR complex with fission yeast Suc22p, although the amino acid sequence identity is only 66% between Rnr1p and Cdc22p.	gene_phenotype
70644	2	334126	7	NULL	NULL	0	NULL	Spd1p	GP		inhibit					Cdc22p activity	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_3_1778_s_90	16317005	To differentiate between inhibition of Suc22p and Cdc22p activity by Spd1p, we took advantage of the observation that budding yeast Rnr1p forms an active RNR complex with fission yeast Suc22p, although the amino acid sequence identity is only 66% between Rnr1p and Cdc22p.	gene_phenotype
70645	3	334126	7	NULL	NULL	0	NULL	Rnr1p	GP	budding yeast	forms complex with					Suc22p	GP	fission yeast 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_3_1778_s_90	16317005	To differentiate between inhibition of Suc22p and Cdc22p activity by Spd1p, we took advantage of the observation that budding yeast Rnr1p forms an active RNR complex with fission yeast Suc22p, although the amino acid sequence identity is only 66% between Rnr1p and Cdc22p.	gene_phenotype
70646	4	334126	7	NULL	NULL	0	NULL	statement 3	Process		is a type of					RNR complex	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_3_1778_s_90	16317005	To differentiate between inhibition of Suc22p and Cdc22p activity by Spd1p, we took advantage of the observation that budding yeast Rnr1p forms an active RNR complex with fission yeast Suc22p, although the amino acid sequence identity is only 66% between Rnr1p and Cdc22p.	gene_phenotype
70649	1	334127	7	NULL	NULL	0	NULL	Spd1	GP		inhibitor of		very weak			RNR	GP	budding yeast			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_3_1778_s_92	16317005	Because Spd1 is a very weak inhibitor of the budding yeast RNR, these results strongly indicate that Spd1 inhibits the fission yeast RNR by specifically interacting with Cdc22p.	gene_phenotype
70650	2	334127	7	NULL	NULL	0	NULL	 Spd1	GP		interact with		specifically			Cdc22p	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_3_1778_s_92	16317005	Because Spd1 is a very weak inhibitor of the budding yeast RNR, these results strongly indicate that Spd1 inhibits the fission yeast RNR by specifically interacting with Cdc22p.	gene_phenotype
70651	3	334127	7	NULL	NULL	0	NULL	Spd1	GP		inhibit					RNR	GP	fission yeast			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_3_1778_s_92	16317005	Because Spd1 is a very weak inhibitor of the budding yeast RNR, these results strongly indicate that Spd1 inhibits the fission yeast RNR by specifically interacting with Cdc22p.	gene_phenotype
70652	4	334127	7	NULL	NULL	0	NULL	statement 3	Process		occur by					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_3_1778_s_92	16317005	Because Spd1 is a very weak inhibitor of the budding yeast RNR, these results strongly indicate that Spd1 inhibits the fission yeast RNR by specifically interacting with Cdc22p.	gene_phenotype
70653	1	334130	7	NULL	NULL	0	NULL	cdt2+	GP	transcription of	fluctuates through					mitotic cell cycle	Process				NULL		0	NULL	NULL	NULL	gw70_genetics_164_3_881_s_128	12871901	As previously reported, transcription of  cdt2+ fluctuates through the mitotic cell cycle with a peak at G1-S phase, similar to the expression pattern of  cdc22+, another target of DSC1 ( Fig 2A).	gene_phenotype
70654	2	334130	7	NULL	NULL	0	NULL	statement 1	Process		peak at					G1-S phase	Process				NULL		0	NULL	NULL	NULL	gw70_genetics_164_3_881_s_128	12871901	As previously reported, transcription of  cdt2+ fluctuates through the mitotic cell cycle with a peak at G1-S phase, similar to the expression pattern of  cdc22+, another target of DSC1 ( Fig 2A).	gene_phenotype
70655	3	334130	7	NULL	NULL	0	NULL	cdt2+	GP	transcription of	is similar to					cdc22+	GP	expression pattern of			NULL		0	NULL	NULL	NULL	gw70_genetics_164_3_881_s_128	12871901	As previously reported, transcription of  cdt2+ fluctuates through the mitotic cell cycle with a peak at G1-S phase, similar to the expression pattern of  cdc22+, another target of DSC1 ( Fig 2A).	gene_phenotype
70656	4	334130	7	NULL	NULL	0	NULL	cdc22+	GP		is target of					DSC1	GP				NULL		0	NULL	NULL	NULL	gw70_genetics_164_3_881_s_128	12871901	As previously reported, transcription of  cdt2+ fluctuates through the mitotic cell cycle with a peak at G1-S phase, similar to the expression pattern of  cdc22+, another target of DSC1 ( Fig 2A).	gene_phenotype
70657	1	334131	7	NULL	NULL	0	NULL	cdc18	GP 	transcription of	is accompanied by					cdc22	GP	mitotic transcription of			NULL		0	NULL	NULL	NULL	gw60_embo_17_19_5689_s_193	9755169	(iii) This  cdc18 transcription is accompanied by the mitotic transcription of other  cdc10-dependent genes, such as  cdc22 and  cdt1, and requires the continued activity of the cdc10p `start'' transcription factor (homologous to the budding yeast Swi6p `start'' transcription factor).	gene_phenotype
70658	2	334131	7	NULL	NULL	0	NULL	cdc18	GP	transcription of	is accompanied by					cdt1	GP	mitotic transcription of			NULL		0	NULL	NULL	NULL	gw60_embo_17_19_5689_s_193	9755169	(iii) This  cdc18 transcription is accompanied by the mitotic transcription of other  cdc10-dependent genes, such as  cdc22 and  cdt1, and requires the continued activity of the cdc10p `start'' transcription factor (homologous to the budding yeast Swi6p `start'' transcription factor).	gene_phenotype
70659	3	334131	7	NULL	NULL	0	NULL	cdc22	GP		is a type of					 cdc10-dependent gene	GP				NULL		0	NULL	NULL	NULL	gw60_embo_17_19_5689_s_193	9755169	(iii) This  cdc18 transcription is accompanied by the mitotic transcription of other  cdc10-dependent genes, such as  cdc22 and  cdt1, and requires the continued activity of the cdc10p `start'' transcription factor (homologous to the budding yeast Swi6p `start'' transcription factor).	gene_phenotype
70660	4	334131	7	NULL	NULL	0	NULL	cdt1	GP		is a type of					cdc10-dependent gene	GP				NULL		0	NULL	NULL	NULL	gw60_embo_17_19_5689_s_193	9755169	(iii) This  cdc18 transcription is accompanied by the mitotic transcription of other  cdc10-dependent genes, such as  cdc22 and  cdt1, and requires the continued activity of the cdc10p `start'' transcription factor (homologous to the budding yeast Swi6p `start'' transcription factor).	gene_phenotype
70661	5	334131	7	NULL	NULL	0	NULL	 cdc18	GP	transcription of	requires					cdc10p `start'' transcription factor	GP	continued activity of			NULL		0	NULL	NULL	NULL	gw60_embo_17_19_5689_s_193	9755169	(iii) This  cdc18 transcription is accompanied by the mitotic transcription of other  cdc10-dependent genes, such as  cdc22 and  cdt1, and requires the continued activity of the cdc10p `start'' transcription factor (homologous to the budding yeast Swi6p `start'' transcription factor).	gene_phenotype
70662	6	334131	7	NULL	NULL	0	NULL	cdc10p `start'' transcription factor	GP		is homologous to					Swi6p `start'' transcription factor	GP	budding yeast			NULL		0	NULL	NULL	NULL	gw60_embo_17_19_5689_s_193	9755169	(iii) This  cdc18 transcription is accompanied by the mitotic transcription of other  cdc10-dependent genes, such as  cdc22 and  cdt1, and requires the continued activity of the cdc10p `start'' transcription factor (homologous to the budding yeast Swi6p `start'' transcription factor).	gene_phenotype
70663	1	334132	7	NULL	NULL	NULL	NULL	DSC1	GP		bind									MCB sequences	NULL		NULL	NULL	NULL	NULL	gw60_embo_21_21_5745_s_19	12411492	DSC1 binds to MCB sequences (  M luI cell  cycle  box; ACGCGT) that are present in the promoters of  cdc22+,  cdc18+,  cdt1+ and  cig2+, all of which are expressed maximally at the G1 - S boundary during the mitotic cell cycle.	gene_phenotype
70664	2	334132	7	NULL	NULL	0	NULL	MCB sequences	GP		present in					cdc22+	GP	promoters of 			NULL		0	NULL	NULL	NULL	gw60_embo_21_21_5745_s_19	12411492	DSC1 binds to MCB sequences (  M luI cell  cycle  box; ACGCGT) that are present in the promoters of  cdc22+,  cdc18+,  cdt1+ and  cig2+, all of which are expressed maximally at the G1 - S boundary during the mitotic cell cycle.	gene_phenotype
70665	3	334132	7	NULL	NULL	0	NULL	MCB sequences	GP		present in					cdc18+	GP	promoters of			NULL		0	NULL	NULL	NULL	gw60_embo_21_21_5745_s_19	12411492	DSC1 binds to MCB sequences (  M luI cell  cycle  box; ACGCGT) that are present in the promoters of  cdc22+,  cdc18+,  cdt1+ and  cig2+, all of which are expressed maximally at the G1 - S boundary during the mitotic cell cycle.	gene_phenotype
70666	4	334132	7	NULL	NULL	0	NULL	MCB sequences 	GP		present in					 cdt1+	GP	promoters of			NULL		0	NULL	NULL	NULL	gw60_embo_21_21_5745_s_19	12411492	DSC1 binds to MCB sequences (  M luI cell  cycle  box; ACGCGT) that are present in the promoters of  cdc22+,  cdc18+,  cdt1+ and  cig2+, all of which are expressed maximally at the G1 - S boundary during the mitotic cell cycle.	gene_phenotype
70667	5	334132	7	NULL	NULL	0	NULL	MCB sequences	GP		present in					cig2+	GP	promoters of			NULL		0	NULL	NULL	NULL	gw60_embo_21_21_5745_s_19	12411492	DSC1 binds to MCB sequences (  M luI cell  cycle  box; ACGCGT) that are present in the promoters of  cdc22+,  cdc18+,  cdt1+ and  cig2+, all of which are expressed maximally at the G1 - S boundary during the mitotic cell cycle.	gene_phenotype
70668	6	334132	7	NULL	NULL	0	NULL	cdc22+	GP		expressed maximally at					G1 - S boundary 	Process				NULL		0	NULL	NULL	NULL	gw60_embo_21_21_5745_s_19	12411492	DSC1 binds to MCB sequences (  M luI cell  cycle  box; ACGCGT) that are present in the promoters of  cdc22+,  cdc18+,  cdt1+ and  cig2+, all of which are expressed maximally at the G1 - S boundary during the mitotic cell cycle.	gene_phenotype
70669	7	334132	7	NULL	NULL	0	NULL	cdc18+	GP		expressed maximally at					G1-S boundary	Process				NULL		0	NULL	NULL	NULL	gw60_embo_21_21_5745_s_19	12411492	DSC1 binds to MCB sequences (  M luI cell  cycle  box; ACGCGT) that are present in the promoters of  cdc22+,  cdc18+,  cdt1+ and  cig2+, all of which are expressed maximally at the G1 - S boundary during the mitotic cell cycle.	gene_phenotype
70670	8	334132	7	NULL	NULL	0	NULL	cdt1+	GP		expressed maximally at					G1-S boundary	Process				NULL		0	NULL	NULL	NULL	gw60_embo_21_21_5745_s_19	12411492	DSC1 binds to MCB sequences (  M luI cell  cycle  box; ACGCGT) that are present in the promoters of  cdc22+,  cdc18+,  cdt1+ and  cig2+, all of which are expressed maximally at the G1 - S boundary during the mitotic cell cycle.	gene_phenotype
70671	9	334132	7	NULL	NULL	0	NULL	cig2+	GP		expressed maximally at					G1-S boundary	Process				NULL		0	NULL	NULL	NULL	gw60_embo_21_21_5745_s_19	12411492	DSC1 binds to MCB sequences (  M luI cell  cycle  box; ACGCGT) that are present in the promoters of  cdc22+,  cdc18+,  cdt1+ and  cig2+, all of which are expressed maximally at the G1 - S boundary during the mitotic cell cycle.	gene_phenotype
70672	10	334132	7	NULL	NULL	0	NULL	statement 6	Process		occur during					mitotic cell cycle	Process				NULL		0	NULL	NULL	NULL	gw60_embo_21_21_5745_s_19	12411492	DSC1 binds to MCB sequences (  M luI cell  cycle  box; ACGCGT) that are present in the promoters of  cdc22+,  cdc18+,  cdt1+ and  cig2+, all of which are expressed maximally at the G1 - S boundary during the mitotic cell cycle.	gene_phenotype
70673	11	334132	7	NULL	NULL	0	NULL	statement 7	Process		occur during					mitotic cell cycle	Process				NULL		0	NULL	NULL	NULL	gw60_embo_21_21_5745_s_19	12411492	DSC1 binds to MCB sequences (  M luI cell  cycle  box; ACGCGT) that are present in the promoters of  cdc22+,  cdc18+,  cdt1+ and  cig2+, all of which are expressed maximally at the G1 - S boundary during the mitotic cell cycle.	gene_phenotype
70674	12	334132	7	NULL	NULL	0	NULL	statement 8	Process		occur during					mitotic cell cycle	Process				NULL		0	NULL	NULL	NULL	gw60_embo_21_21_5745_s_19	12411492	DSC1 binds to MCB sequences (  M luI cell  cycle  box; ACGCGT) that are present in the promoters of  cdc22+,  cdc18+,  cdt1+ and  cig2+, all of which are expressed maximally at the G1 - S boundary during the mitotic cell cycle.	gene_phenotype
70675	13	334132	7	NULL	NULL	0	NULL	statement 9	Process		occur during					mitotic cell cycle	Process				NULL		0	NULL	NULL	NULL	gw60_embo_21_21_5745_s_19	12411492	DSC1 binds to MCB sequences (  M luI cell  cycle  box; ACGCGT) that are present in the promoters of  cdc22+,  cdc18+,  cdt1+ and  cig2+, all of which are expressed maximally at the G1 - S boundary during the mitotic cell cycle.	gene_phenotype
70676	14	334132	7	NULL	NULL	0	NULL	MCB sequences 	GP		is					M luI cell cycle box; ACGCGT	GP				NULL		0	NULL	NULL	NULL	gw60_embo_21_21_5745_s_19	12411492	DSC1 binds to MCB sequences (  M luI cell  cycle  box; ACGCGT) that are present in the promoters of  cdc22+,  cdc18+,  cdt1+ and  cig2+, all of which are expressed maximally at the G1 - S boundary during the mitotic cell cycle.	gene_phenotype
70677	1	334133	7	NULL	NULL	NULL	NULL	mik1+ transcript	GP	abundance of	coincides with					cdc22+ transcript	GP	abundance of			NULL	wild-type cells	NULL	NULL	NULL	NULL	gw60_febslett_503_2_131_s_67	11513869	In a synchronous population of wild-type cells, size selected by elutriation,  mik1+ transcript was found to vary in abundance ( Fig. 1B) coincident with  cdc22+ transcript, thus peaking at the G1-S boundary.	gene_phenotype
70678	2	334133	7	NULL	NULL	0	NULL	statement 1	Process		peaks at					G1-S boundary	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_503_2_131_s_67	11513869	In a synchronous population of wild-type cells, size selected by elutriation,  mik1+ transcript was found to vary in abundance ( Fig. 1B) coincident with  cdc22+ transcript, thus peaking at the G1-S boundary.	gene_phenotype
70679	1	334135	7	NULL	NULL	0	NULL	cdc18	GP		required for					DNA replication	Process				NULL		0	NULL	NULL	NULL	gw60_nature_409_6818_359_s_30	11201746	Two genes required for DNA replication,  cdc18 and  cdc22, were induced only during G1-exit meiosis ( Fig. 1c), which was consistent with the fact that G2-exit meiotic cells do not undergo a pre-meiotic S phase.	gene_phenotype
70680	2	334135	7	NULL	NULL	0	NULL	cdc22	GP		required for					DNA replication	Process				NULL		0	NULL	NULL	NULL	gw60_nature_409_6818_359_s_30	11201746	Two genes required for DNA replication,  cdc18 and  cdc22, were induced only during G1-exit meiosis ( Fig. 1c), which was consistent with the fact that G2-exit meiotic cells do not undergo a pre-meiotic S phase.	gene_phenotype
70681	3	334135	7	NULL	NULL	0	NULL	statement 1	Process		induced at					G1-exit meiosis	Process				NULL		0	NULL	NULL	NULL	gw60_nature_409_6818_359_s_30	11201746	Two genes required for DNA replication,  cdc18 and  cdc22, were induced only during G1-exit meiosis ( Fig. 1c), which was consistent with the fact that G2-exit meiotic cells do not undergo a pre-meiotic S phase.	gene_phenotype
70682	4	334135	7	NULL	NULL	NULL	NULL	statement 2	Process		induced at					G1-exit meiosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_nature_409_6818_359_s_30	11201746	Two genes required for DNA replication,  cdc18 and  cdc22, were induced only during G1-exit meiosis ( Fig. 1c), which was consistent with the fact that G2-exit meiotic cells do not undergo a pre-meiotic S phase.	gene_phenotype
70683	5	334135	7	NULL	NULL	0	NULL	G2-exit meiotic cells	Cell		does not undergo					pre-meiotic S phase	Process				NULL		0	NULL	NULL	NULL	gw60_nature_409_6818_359_s_30	11201746	Two genes required for DNA replication,  cdc18 and  cdc22, were induced only during G1-exit meiosis ( Fig. 1c), which was consistent with the fact that G2-exit meiotic cells do not undergo a pre-meiotic S phase.	gene_phenotype
70684	1	334136	7	NULL	NULL	0	NULL	cdc22+ gene	GP	Schizosaccharomyces pombe	encode					ribonucleotide reductase	GP		large subunit of		NULL		0	NULL	NULL	NULL	abs-batch0517-0529_mol-genet-genomics_269_6_12898217_s_2	12898217	The cdc22+ gene of the fission yeast, Schizosaccharomyces pombe, encodes  the large subunit of ribonucleotide reductase, and is periodically expressed  during the mitotic cell cycle, transcript abundance reaching a maximum  at the G1-S boundary.	gene_phenotype
70685	2	334136	7	NULL	NULL	0	NULL	statement 1	Process		expressed during		periodically			mitotic cell cycle	Process				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_mol-genet-genomics_269_6_12898217_s_2	12898217	The cdc22+ gene of the fission yeast, Schizosaccharomyces pombe, encodes  the large subunit of ribonucleotide reductase, and is periodically expressed  during the mitotic cell cycle, transcript abundance reaching a maximum  at the G1-S boundary.	gene_phenotype
70686	3	334136	7	NULL	NULL	0	NULL	cdc22+ transcript	GP	abundance of	reaches 					G1-S boundary	Process	maximum at			NULL		0	NULL	NULL	NULL	abs-batch0517-0529_mol-genet-genomics_269_6_12898217_s_2	12898217	The cdc22+ gene of the fission yeast, Schizosaccharomyces pombe, encodes  the large subunit of ribonucleotide reductase, and is periodically expressed  during the mitotic cell cycle, transcript abundance reaching a maximum  at the G1-S boundary.	gene_phenotype
70687	4	334136	7	NULL	NULL	0	NULL	Schizosaccharomyces pombe	Organism		is a type of					fission yeast	Organism				NULL		0	NULL	NULL	NULL	abs-batch0517-0529_mol-genet-genomics_269_6_12898217_s_2	12898217	The cdc22+ gene of the fission yeast, Schizosaccharomyces pombe, encodes  the large subunit of ribonucleotide reductase, and is periodically expressed  during the mitotic cell cycle, transcript abundance reaching a maximum  at the G1-S boundary.	gene_phenotype
70688	1	334137	7	NULL	NULL	0	NULL	Sml1	GP		bind					Rnr1p	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_3_1778_s_28	16317005	This mode of regulation is similar to the regulation of RNR activity in budding yeast, where binding of the low molecular weight inhibitor Sml1 to the Cdc22p homologue, the Rnr1p, controls RNR activity.	gene_phenotype
70689	2	334137	7	NULL	NULL	NULL	NULL	statement 1	Process		controls					RNR activity	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_3_1778_s_28	16317005	This mode of regulation is similar to the regulation of RNR activity in budding yeast, where binding of the low molecular weight inhibitor Sml1 to the Cdc22p homologue, the Rnr1p, controls RNR activity.	gene_phenotype
70690	3	334137	7	NULL	NULL	0	NULL	Rnr1p	GP		is homologous to					Cdc22p	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_3_1778_s_28	16317005	This mode of regulation is similar to the regulation of RNR activity in budding yeast, where binding of the low molecular weight inhibitor Sml1 to the Cdc22p homologue, the Rnr1p, controls RNR activity.	gene_phenotype
70691	4	334137	7	NULL	NULL	0	NULL	Sml1	GP		is a type of					low molecular weight inhibitor	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_3_1778_s_28	16317005	This mode of regulation is similar to the regulation of RNR activity in budding yeast, where binding of the low molecular weight inhibitor Sml1 to the Cdc22p homologue, the Rnr1p, controls RNR activity.	gene_phenotype
70692	5	334137	7	NULL	NULL	0	NULL	statement 1	Process		occur in					budding yeast	Organism				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_3_1778_s_28	16317005	This mode of regulation is similar to the regulation of RNR activity in budding yeast, where binding of the low molecular weight inhibitor Sml1 to the Cdc22p homologue, the Rnr1p, controls RNR activity.	gene_phenotype
70693	1	334138	7	NULL	NULL	0	NULL	Spd1p	GP		interacts with					Cdc22p	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_3_1778_s_56	16317005	The interaction between Spd1p and Cdc22p, Suc22p, budding yeast Rnr1p, Sml1p, and mouse R1 protein was studied by biosensor analysis using a BIAcore 2000 (Biacore International AB).	gene_phenotype
70694	2	334138	7	NULL	NULL	0	NULL	Spd1p	GP		interacts with					Suc22p	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_3_1778_s_56	16317005	The interaction between Spd1p and Cdc22p, Suc22p, budding yeast Rnr1p, Sml1p, and mouse R1 protein was studied by biosensor analysis using a BIAcore 2000 (Biacore International AB).	gene_phenotype
70695	3	334138	7	NULL	NULL	0	NULL	Spd1p	GP		interacts with					 Rnr1p	GP	budding yeast			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_3_1778_s_56	16317005	The interaction between Spd1p and Cdc22p, Suc22p, budding yeast Rnr1p, Sml1p, and mouse R1 protein was studied by biosensor analysis using a BIAcore 2000 (Biacore International AB).	gene_phenotype
70696	4	334138	7	NULL	NULL	0	NULL	Spd1p	GP		interacts with					Sml1p	GP	budding yeast			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_3_1778_s_56	16317005	The interaction between Spd1p and Cdc22p, Suc22p, budding yeast Rnr1p, Sml1p, and mouse R1 protein was studied by biosensor analysis using a BIAcore 2000 (Biacore International AB).	gene_phenotype
70697	5	334138	7	NULL	NULL	0	NULL	Spd1p	GP		interacts with					R1 protein	GP	mouse			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_3_1778_s_56	16317005	The interaction between Spd1p and Cdc22p, Suc22p, budding yeast Rnr1p, Sml1p, and mouse R1 protein was studied by biosensor analysis using a BIAcore 2000 (Biacore International AB).	gene_phenotype
70698	1	334139	7	NULL	NULL	NULL	NULL	Spd1p	GP		inhibit					Cdc22p plus Suc22p	GP	recombinant			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_3_1778_s_87	16317005	Inhibition by Spd1p -- Recombinant Cdc22p plus Suc22p was assayed for activity using the CDP reduction assay, with ATP as a positive effector in the presence of increasing amounts of Spd1 protein ( Fig. 2).	gene_phenotype
70700	1	334140	7	NULL	NULL	0	NULL	Spd1 protein	GP		inhibit		very little			Rnr1p plus Suc22p	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_3_1778_s_91	16317005	Assaying recombinant budding yeast Rnr1p plus Suc22p for activity using the CDP reduction assay in the presence of increasing amounts of Spd1 protein showed very little inhibition compared with the results with Cdc22p and Suc22p ( Fig. 2).	gene_phenotype
70701	1	334141	7	NULL	NULL	0	NULL	DSC1	GP		control					cdc22+ genes	GP				NULL		0	NULL	NULL	NULL	gw60_embo_21_21_5745_s_278	12411492	There is precedence in fission yeast for groups of genes being regulated by a similar transcription factor complex in both mitosis and meiosis: DSC1 and MCB sequences control  cdc22+ and the  rec+ genes during the two life cycles (L.Cunliffe, S.White and C.J.McInerny, unpublished data).	gene_phenotype
70702	2	334141	7	NULL	NULL	0	NULL	DSC1	GP		control					 rec+ genes	GP				NULL		0	NULL	NULL	NULL	gw60_embo_21_21_5745_s_278	12411492	There is precedence in fission yeast for groups of genes being regulated by a similar transcription factor complex in both mitosis and meiosis: DSC1 and MCB sequences control  cdc22+ and the  rec+ genes during the two life cycles (L.Cunliffe, S.White and C.J.McInerny, unpublished data).	gene_phenotype
70703	3	334141	7	NULL	NULL	NULL	NULL				control				MCB sequences	cdc22+ genes	GP				NULL		NULL	NULL	NULL	NULL	gw60_embo_21_21_5745_s_278	12411492	There is precedence in fission yeast for groups of genes being regulated by a similar transcription factor complex in both mitosis and meiosis: DSC1 and MCB sequences control  cdc22+ and the  rec+ genes during the two life cycles (L.Cunliffe, S.White and C.J.McInerny, unpublished data).	gene_phenotype
70704	4	334141	7	NULL	NULL	0	NULL				control				MCB sequences	rec+ genes	GP				NULL		0	NULL	NULL	NULL	gw60_embo_21_21_5745_s_278	12411492	There is precedence in fission yeast for groups of genes being regulated by a similar transcription factor complex in both mitosis and meiosis: DSC1 and MCB sequences control  cdc22+ and the  rec+ genes during the two life cycles (L.Cunliffe, S.White and C.J.McInerny, unpublished data).	gene_phenotype
70705	5	334141	7	NULL	NULL	0	NULL	statement 3	Process		occur during					lifecycle	Process				NULL		0	NULL	NULL	NULL	gw60_embo_21_21_5745_s_278	12411492	There is precedence in fission yeast for groups of genes being regulated by a similar transcription factor complex in both mitosis and meiosis: DSC1 and MCB sequences control  cdc22+ and the  rec+ genes during the two life cycles (L.Cunliffe, S.White and C.J.McInerny, unpublished data).	gene_phenotype
70706	6	334141	7	NULL	NULL	0	NULL	statement 4	Process		occur during					lifecycle	Process				NULL		0	NULL	NULL	NULL	gw60_embo_21_21_5745_s_278	12411492	There is precedence in fission yeast for groups of genes being regulated by a similar transcription factor complex in both mitosis and meiosis: DSC1 and MCB sequences control  cdc22+ and the  rec+ genes during the two life cycles (L.Cunliffe, S.White and C.J.McInerny, unpublished data).	gene_phenotype
70707	1	334143	7	NULL	NULL	0	NULL	YML083c	GP		shows					higher transcript levels 	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_5_439_s_57	12673627	YML083c and  DAN1 exhibited 29- and 40-fold higher transcript levels during anaerobic growth respectively  (Ter Linde  et al., [ 1999]).	gene_phenotype
70708	2	334143	7	NULL	NULL	0	NULL	DAN1 	GP		shows					higher transcript levels 	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_5_439_s_57	12673627	YML083c and  DAN1 exhibited 29- and 40-fold higher transcript levels during anaerobic growth respectively  (Ter Linde  et al., [ 1999]).	gene_phenotype
70709	3	334143	7	NULL	NULL	0	NULL	statement 1	Process		during					anaerobic growth	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_5_439_s_57	12673627	YML083c and  DAN1 exhibited 29- and 40-fold higher transcript levels during anaerobic growth respectively  (Ter Linde  et al., [ 1999]).	gene_phenotype
70710	4	334143	7	NULL	NULL	0	NULL	statement 2	Process		during					anaerobic growth	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_5_439_s_57	12673627	YML083c and  DAN1 exhibited 29- and 40-fold higher transcript levels during anaerobic growth respectively  (Ter Linde  et al., [ 1999]).	gene_phenotype
70711	1	334144	7	NULL	NULL	0	NULL	YML083c protein	GP		plays					sterols	Chemical	non-essential role in transport of			NULL		0	NULL	NULL	NULL	gw70_yeast_20_5_439_s_421	12673627	It is possible that the YML083c protein plays a non-essential role in the transport  of sterols, as suggested by the fact that regulation by Upc2 affects control of this  process (Crowley  et al., [ 1998]).	gene_phenotype
70712	2	334144	7	NULL	NULL	0	NULL	Upc2	GP	regulation by	controls					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_5_439_s_421	12673627	It is possible that the YML083c protein plays a non-essential role in the transport  of sterols, as suggested by the fact that regulation by Upc2 affects control of this  process (Crowley  et al., [ 1998]).	gene_phenotype
70713	3	334144	7	NULL	NULL	0	NULL	statement 2	Process		suggests					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_5_439_s_421	12673627	It is possible that the YML083c protein plays a non-essential role in the transport  of sterols, as suggested by the fact that regulation by Upc2 affects control of this  process (Crowley  et al., [ 1998]).	gene_phenotype
70714	1	334145	7	NULL	NULL	0	NULL	YML083c	GP		is a type of					ORFs	GP	Saccharomyces cerevisiae			NULL		0	NULL	NULL	NULL	gw70_yeast_20_5_439_s_2	12673627	YML083c and  DAN1 were among the  Saccharomyces cerevisiae ORFs that displayed the strongest increase in transcript abundance during anaerobic  growth compared to aerobic growth, as determined by oligonucleotide microarrays.	gene_phenotype
70715	2	334145	7	NULL	NULL	0	NULL	DAN1	GP		is a type of					ORFs	GP	Saccharomyces cerevisiae			NULL		0	NULL	NULL	NULL	gw70_yeast_20_5_439_s_2	12673627	YML083c and  DAN1 were among the  Saccharomyces cerevisiae ORFs that displayed the strongest increase in transcript abundance during anaerobic  growth compared to aerobic growth, as determined by oligonucleotide microarrays.	gene_phenotype
70716	3	334145	7	NULL	NULL	NULL	NULL	statement 1	Process		displays					transcript	NucleicAcid	 increase in abundance of			NULL		NULL	NULL	NULL	NULL	gw70_yeast_20_5_439_s_2	12673627	YML083c and  DAN1 were among the  Saccharomyces cerevisiae ORFs that displayed the strongest increase in transcript abundance during anaerobic  growth compared to aerobic growth, as determined by oligonucleotide microarrays.	gene_phenotype
70717	4	334145	7	NULL	NULL	NULL	NULL	statement 2	Process		displays					transcript	NucleicAcid	increase in abundance of			NULL		NULL	NULL	NULL	NULL	gw70_yeast_20_5_439_s_2	12673627	YML083c and  DAN1 were among the  Saccharomyces cerevisiae ORFs that displayed the strongest increase in transcript abundance during anaerobic  growth compared to aerobic growth, as determined by oligonucleotide microarrays.	gene_phenotype
70718	5	334145	7	NULL	NULL	0	NULL	statement 3	Process		occur during					aerobic growth	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_5_439_s_2	12673627	YML083c and  DAN1 were among the  Saccharomyces cerevisiae ORFs that displayed the strongest increase in transcript abundance during anaerobic  growth compared to aerobic growth, as determined by oligonucleotide microarrays.	gene_phenotype
70719	6	334145	7	NULL	NULL	0	NULL	statement 3	Process		occur during					anaerobic growth	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_5_439_s_2	12673627	YML083c and  DAN1 were among the  Saccharomyces cerevisiae ORFs that displayed the strongest increase in transcript abundance during anaerobic  growth compared to aerobic growth, as determined by oligonucleotide microarrays.	gene_phenotype
70720	7	334145	7	NULL	NULL	0	NULL	statement 4	Process		occur during					aerobic growth	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_5_439_s_2	12673627	YML083c and  DAN1 were among the  Saccharomyces cerevisiae ORFs that displayed the strongest increase in transcript abundance during anaerobic  growth compared to aerobic growth, as determined by oligonucleotide microarrays.	gene_phenotype
70721	8	334145	7	NULL	NULL	0	NULL	statement 4	Process		occur during					anaerobic growth	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_5_439_s_2	12673627	YML083c and  DAN1 were among the  Saccharomyces cerevisiae ORFs that displayed the strongest increase in transcript abundance during anaerobic  growth compared to aerobic growth, as determined by oligonucleotide microarrays.	gene_phenotype
70722	9	334145	7	NULL	NULL	0	NULL	statement 6	Process		is stronger than					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_5_439_s_2	12673627	YML083c and  DAN1 were among the  Saccharomyces cerevisiae ORFs that displayed the strongest increase in transcript abundance during anaerobic  growth compared to aerobic growth, as determined by oligonucleotide microarrays.	gene_phenotype
70723	10	334145	7	NULL	NULL	0	NULL	statement 8	Process		is stronger than					statement 7	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_20_5_439_s_2	12673627	YML083c and  DAN1 were among the  Saccharomyces cerevisiae ORFs that displayed the strongest increase in transcript abundance during anaerobic  growth compared to aerobic growth, as determined by oligonucleotide microarrays.	gene_phenotype
70724	1	334146	7	NULL	NULL	0	NULL	mRNA 	NucleicAcid		shows					anaerobic growth	Process	higher level during			NULL		0	NULL	NULL	NULL	gw70_yeast_20_5_439_s_200	12673627	The behaviour of the full-length YML083c promoter- lacZ fusion borne on a single-copy plasmid was consistent with the microarray data, which  indicated a much higher mRNA level during anaerobic growth.	gene_phenotype
70725	2	334146	7	NULL	NULL	NULL	NULL	YML083c	GP	behaviour of;;full-length	indicates				promoter	statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_yeast_20_5_439_s_200	12673627	The behaviour of the full-length YML083c promoter- lacZ fusion borne on a single-copy plasmid was consistent with the microarray data, which  indicated a much higher mRNA level during anaerobic growth.	gene_phenotype
70726	1	334147	7	NULL	NULL	0	NULL	Mpr1p	GP	purified;;recombinant E. coli cells	acetylates					AZC	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_45_41998_s_166	11555637	AZC Acetylation by Mpr1p-- The His-tagged fusion Mpr1p was purified from the recombinant  E. coli cells expressing the  MPR1 gene as described under	gene_phenotype
70727	1	334148	7	NULL	NULL	NULL	NULL	Sporulation	Process		generates					mpr1::his7+ spc1::ura4+	Chromosome	viable  haploid segregants of			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_66	10749922	Sporulation and tetrad dissection generated viable haploid segregants of  mpr1::his7+ spc1::ura4+ and  mpr1::his7+ spc1+, which indicated that  mpr1+ is not essential for cellular viability.	gene_phenotype
70728	2	334148	7	NULL	NULL	NULL	NULL	tetrad dissection	Process		generates					mpr1::his7+ spc1+	Chromosome	viable haploid segregants of			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_66	10749922	Sporulation and tetrad dissection generated viable haploid segregants of  mpr1::his7+ spc1::ura4+ and  mpr1::his7+ spc1+, which indicated that  mpr1+ is not essential for cellular viability.	gene_phenotype
70729	3	334148	7	NULL	NULL	0	NULL	mpr1+	GP		is not essential for					cellular viability	Process				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_66	10749922	Sporulation and tetrad dissection generated viable haploid segregants of  mpr1::his7+ spc1::ura4+ and  mpr1::his7+ spc1+, which indicated that  mpr1+ is not essential for cellular viability.	gene_phenotype
70730	1	334150	7	NULL	NULL	NULL	NULL				is essential for			 conserved phosphorylation site His-221		Mpr1 function	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_48	10749922	In addition, the conserved phosphorylation site, His-221, is essential for Mpr1 function, and Mpr1 binds to the Mcs4 response regulator in response to oxidative stress.	gene_phenotype
70731	2	334150	7	NULL	NULL	0	NULL	Mpr1	GP		bind					Mcs4 response regulator	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_48	10749922	In addition, the conserved phosphorylation site, His-221, is essential for Mpr1 function, and Mpr1 binds to the Mcs4 response regulator in response to oxidative stress.	gene_phenotype
70732	3	334150	7	NULL	NULL	0	NULL	statement 2	Process		in response to					oxidative stress	Process				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_48	10749922	In addition, the conserved phosphorylation site, His-221, is essential for Mpr1 function, and Mpr1 binds to the Mcs4 response regulator in response to oxidative stress.	gene_phenotype
70733	1	334151	7	NULL	NULL	0	NULL	Mpr1 	GP		is homologous to					Ypd1	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_94	10749922	Mpr1 Is Homologous to Ypd1, a Response Regulator Phosphotransferase in Budding Yeast	gene_phenotype
70734	2	334151	7	NULL	NULL	0	NULL	Ypd1	GP		is a type of					Response Regulator Phosphotransferase					NULL	budding yeast	0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_94	10749922	Mpr1 Is Homologous to Ypd1, a Response Regulator Phosphotransferase in Budding Yeast	gene_phenotype
70735	1	334152	7	NULL	NULL	0	NULL	Mpr1	GP		is crucial for			Putative Histidine Phosphorylation Site		Oxidative Stress Signaling	Process				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_136	10749922	The Putative Histidine Phosphorylation Site of Mpr1 Is Crucial for Oxidative Stress Signaling	gene_phenotype
70736	1	334153	7	NULL	NULL	0	NULL	Mpr1	GP	fission yeast	is homologous to					Ypd1 response regulator phosphotransferase	GP	budding yeast			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_20_17722_s_17	11886858	Fission yeast Mpr1 is homologous to the Ypd1 response regulator phosphotransferase in budding yeast.	gene_phenotype
70737	1	334154	7	NULL	NULL	0	NULL	Mpr1 	GP		combines with					l-proline	AminoAcid				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_j-biochem-(tokyo)_138_4_16272133_s_5	16272133	The combination of  Mpr1 and l-proline could further enhance the resistance to freezing stress.	gene_phenotype
70738	2	334154	7	NULL	NULL	0	NULL	statement 1	Process		enhance					freezing stress	Process	resistance to			NULL		0	NULL	NULL	NULL	abs-batch0540-0549_j-biochem-(tokyo)_138_4_16272133_s_5	16272133	The combination of  Mpr1 and l-proline could further enhance the resistance to freezing stress.	gene_phenotype
70740	1	334156	7	NULL	NULL	NULL	NULL	Mpr1	GP		is conserved between			His-221 phosphorylation site		 Ypd1	GP		His-221 phosphorylation site		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_137	10749922	Sequence conservation of the histidine phosphorylation site between Mpr1 and Ypd1 (Figure  1A) prompted us to test whether phosphorylation of His-221 in Mpr1 is required for oxidative stress signaling.	gene_phenotype
70741	1	334157	7	NULL	NULL	0	NULL	MPR1	GP	overexpression of	leads to					cell viability	Process	increase in			NULL		0	NULL	NULL	NULL	gw70_pnas_101_34_12616_s_5	15308773	In contrast, overexpression of  MPR1 leads to an increase in cell viability and a decrease in ROS level after oxidative treatments.	gene_phenotype
70742	2	334157	7	NULL	NULL	0	NULL	MPR1	GP	overexpression of	decrease					ROS level	Chemical				NULL		0	NULL	NULL	NULL	gw70_pnas_101_34_12616_s_5	15308773	In contrast, overexpression of  MPR1 leads to an increase in cell viability and a decrease in ROS level after oxidative treatments.	gene_phenotype
70743	3	334157	7	NULL	NULL	0	NULL	statement 1	Process		occur after					oxidative treatment	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_101_34_12616_s_5	15308773	In contrast, overexpression of  MPR1 leads to an increase in cell viability and a decrease in ROS level after oxidative treatments.	gene_phenotype
70744	4	334157	7	NULL	NULL	0	NULL	statement 2	Process		occur after					oxidative treatment	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_101_34_12616_s_5	15308773	In contrast, overexpression of  MPR1 leads to an increase in cell viability and a decrease in ROS level after oxidative treatments.	gene_phenotype
70745	1	334158	7	NULL	NULL	0	NULL	 MPR genes	GP	null mutant	displays					hypersensitivity	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_101_34_12616_s_254	15308773	In summary, the null mutant of the  MPR genes displayed hypersensitivity to oxidative stress, and the expression of the  MPR1 gene conferred stress resistance.	gene_phenotype
70746	2	334158	7	NULL	NULL	0	NULL	statement 1	Process		in response to					oxidative stress	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_101_34_12616_s_254	15308773	In summary, the null mutant of the  MPR genes displayed hypersensitivity to oxidative stress, and the expression of the  MPR1 gene conferred stress resistance.	gene_phenotype
70747	3	334158	7	NULL	NULL	0	NULL	MPR1 gene 	GP	expression of	confers					stress	Process	resistance to			NULL		0	NULL	NULL	NULL	gw70_pnas_101_34_12616_s_254	15308773	In summary, the null mutant of the  MPR genes displayed hypersensitivity to oxidative stress, and the expression of the  MPR1 gene conferred stress resistance.	gene_phenotype
70748	1	334159	7	NULL	NULL	0	NULL	mpr1+ gene	GP	fission yeast	encode					novel protein	GP		histidine-containing phosphotransfer domain 		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_4	10749922	The fission yeast  mpr1+ gene encodes a novel protein with a histidine-containing phosphotransfer domain homologous to the budding yeast Ypd1.	gene_phenotype
70749	2	334159	7	NULL	NULL	0	NULL	novel protein	GP		is homologous to			histidine-containing phosphotransfer domain 		Ypd1	GP	budding yeast			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_4	10749922	The fission yeast  mpr1+ gene encodes a novel protein with a histidine-containing phosphotransfer domain homologous to the budding yeast Ypd1.	gene_phenotype
70750	1	334160	7	NULL	NULL	0	NULL	Mpr1	GP	fission yeast	homologous to		highly			Ypd1 response regulator phosphotransferase	GP	budding yeast			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_46	10749922	In this report, we have characterized the fission yeast Mpr1, which is highly homologous to the Ypd1 response regulator phosphotransferase in budding yeast.	gene_phenotype
70751	1	334161	7	NULL	NULL	0	NULL	Mpr1 	GP	fission yeast	is homologous to					Ypd1 protein	GP	budding yeast			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_103	10749922	Mpr1 is a fission yeast homologue of the budding yeast Ypd1 protein, a response regulator phosphotransferase.	gene_phenotype
70752	2	334161	7	NULL	NULL	0	NULL	Ypd1 protein	GP		is a type of					response regulator phosphotransferase	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_103	10749922	Mpr1 is a fission yeast homologue of the budding yeast Ypd1 protein, a response regulator phosphotransferase.	gene_phenotype
70754	1	334162	7	NULL	NULL	NULL	NULL	Mpr1	GP		is required for			putative phosphorylation site His-221		oxidative stress signaling 	Process	function in			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_143	10749922	These results indicate that the putative phosphorylation site, His-221, is required for the Mpr1 function in oxidative stress signaling to Spc1.	gene_phenotype
70766	1	334165	7	NULL	NULL	0	NULL	AZC resistance strain	Organism		produce					Mpr1 proteins	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_45_41998_s_143	11555637	AZC resistance and acetylation activity in the strains producing the various Mpr1 proteins correlated with each other.	gene_phenotype
70767	2	334165	7	NULL	NULL	0	NULL	acetylation activity in the strains	Process		produce					Mpr1 proteins	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_45_41998_s_143	11555637	AZC resistance and acetylation activity in the strains producing the various Mpr1 proteins correlated with each other.	gene_phenotype
70771	1	334166	7	NULL	NULL	0	NULL	ASA	Chemical		converted to					 L-azetidine-2-carboxylic acid	Chemical				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_3_5_1287_s_229	15470257	A plasmid expressing  MPR1 did not rescue viability of  fpr1delta hom6delta double mutants, suggesting that ASA conversion into L-azetidine-2-carboxylic acid is not the basis for ASA toxicity.	gene_phenotype
70772	2	334166	7	NULL	NULL	0	NULL	statement 1	Process		is not the basis for					ASA toxicity	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_3_5_1287_s_229	15470257	A plasmid expressing  MPR1 did not rescue viability of  fpr1delta hom6delta double mutants, suggesting that ASA conversion into L-azetidine-2-carboxylic acid is not the basis for ASA toxicity.	gene_phenotype
70926	1	334167	7	NULL	NULL	NULL	NULL	 CKY8	Organism		carries					MPR1	GP				NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_34_12616_s_121	15308773	In contrast, overexpression of  MPR1 in strain CKY8 showed a 3-fold higher cell viability compared with that of strain CKY8 carrying only the vector against heat shock.	gene_phenotype
70928	2	334167	7	NULL	NULL	0	NULL	CKY8	Organism		carries					heat shock	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_34_12616_s_121	15308773	In contrast, overexpression of  MPR1 in strain CKY8 showed a 3-fold higher cell viability compared with that of strain CKY8 carrying only the vector against heat shock.	gene_phenotype
70931	3	334167	7	NULL	NULL	0	NULL	statement 1	Process	cell viability of	is higher  than					statement 2	Process	cell viability of			NULL		0	NULL	NULL	NULL	gw70_pnas_101_34_12616_s_121	15308773	In contrast, overexpression of  MPR1 in strain CKY8 showed a 3-fold higher cell viability compared with that of strain CKY8 carrying only the vector against heat shock.	gene_phenotype
70932	1	334168	7	NULL	NULL	0	NULL	Saccharomyces cerevisiae	Organism	budding yeast	encode					uncharacterized N-acetyltransferase	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_34_12616_s_2	15308773	he  MPR1 gene, which is found in the sigma1278b strain but is not present in the sequenced laboratory strain S288C, of the budding yeast  Saccharomyces cerevisiae encodes a previously uncharacterized  N-acetyltransferase that detoxifies the proline analogue azetidine-2-carboxylate (AZC).	gene_phenotype
70933	2	334168	7	NULL	NULL	0	NULL	statement 1	GP		detoxifies					AZC	Chemical				NULL		0	NULL	NULL	NULL	gw70_pnas_101_34_12616_s_2	15308773	he  MPR1 gene, which is found in the sigma1278b strain but is not present in the sequenced laboratory strain S288C, of the budding yeast  Saccharomyces cerevisiae encodes a previously uncharacterized  N-acetyltransferase that detoxifies the proline analogue azetidine-2-carboxylate (AZC).	gene_phenotype
70934	3	334168	7	NULL	NULL	0	NULL	AZC	Chemical		is					azetidine-2-carboxylate	Chemical				NULL		0	NULL	NULL	NULL	gw70_pnas_101_34_12616_s_2	15308773	he  MPR1 gene, which is found in the sigma1278b strain but is not present in the sequenced laboratory strain S288C, of the budding yeast  Saccharomyces cerevisiae encodes a previously uncharacterized  N-acetyltransferase that detoxifies the proline analogue azetidine-2-carboxylate (AZC).	gene_phenotype
70935	4	334168	7	NULL	NULL	0	NULL	AZC	Chemical		is a type of					proline analogue	Chemical				NULL		0	NULL	NULL	NULL	gw70_pnas_101_34_12616_s_2	15308773	he  MPR1 gene, which is found in the sigma1278b strain but is not present in the sequenced laboratory strain S288C, of the budding yeast  Saccharomyces cerevisiae encodes a previously uncharacterized  N-acetyltransferase that detoxifies the proline analogue azetidine-2-carboxylate (AZC).	gene_phenotype
70936	1	334169	7	NULL	NULL	0	NULL	mpr1+	GP		is not essential for					viability	Process				NULL	spc1+ background	0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_118	10749922	All of the dissected tetrads gave rise to four viable spores with 2:2 segregation of His+ and His  phenotypes regardless of the uracil auxotrophy, indicating that  mpr1+ is not essential for viability in both  spc1+ and  spc1  backgrounds.	gene_phenotype
70937	2	334169	7	NULL	NULL	NULL	NULL	mpr1+	GP		is not essential for					viability	Process				NULL	spc1 background	NULL	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_118	10749922	All of the dissected tetrads gave rise to four viable spores with 2:2 segregation of His+ and His  phenotypes regardless of the uracil auxotrophy, indicating that  mpr1+ is not essential for viability in both  spc1+ and  spc1  backgrounds.	gene_phenotype
70938	1	334170	7	NULL	NULL	NULL	NULL	oxidative stress signaling 	Process		in response to					Spc1 SAPK cascade	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_129	10749922	These results implicate Mpr1 in oxidative stress signaling to the Spc1 SAPK cascade, which contrasts with the function of Ypd1 in osmostress signaling of budding yeast (Posas  et al., 1996  ).	gene_phenotype
70939	2	334170	7	NULL	NULL	0	NULL	Ypd1	GP	function of	in response to					osmostress signaling	Process	budding yeast			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_129	10749922	These results implicate Mpr1 in oxidative stress signaling to the Spc1 SAPK cascade, which contrasts with the function of Ypd1 in osmostress signaling of budding yeast (Posas  et al., 1996  ).	gene_phenotype
70940	4	334170	7	NULL	NULL	NULL	NULL	statement 3	Process		in contrast to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_129	10749922	These results implicate Mpr1 in oxidative stress signaling to the Spc1 SAPK cascade, which contrasts with the function of Ypd1 in osmostress signaling of budding yeast (Posas  et al., 1996  ).	gene_phenotype
70941	3	334170	7	NULL	NULL	0	NULL	 Mpr1	GP		implicated in					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_129	10749922	These results implicate Mpr1 in oxidative stress signaling to the Spc1 SAPK cascade, which contrasts with the function of Ypd1 in osmostress signaling of budding yeast (Posas  et al., 1996  ).	gene_phenotype
70942	1	334171	7	NULL	NULL	0	NULL	Mpr1	GP		is most homologous to					Ypd1 protein	GP	budding yeast			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_273	10749922	Mpr1 is most homologous to the budding yeast Ypd1 protein, which transfers a phosphoryl group from the receiver domain of Sln1 to the Ssk1 response regulator in osmostress signaling to the Hog1 MAPK cascade.	gene_phenotype
70943	2	334171	7	NULL	NULL	0	NULL	Sln1	GP		transferred to			phosphoryl group from the receiver domain		Ssk1 response regulator	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_273	10749922	Mpr1 is most homologous to the budding yeast Ypd1 protein, which transfers a phosphoryl group from the receiver domain of Sln1 to the Ssk1 response regulator in osmostress signaling to the Hog1 MAPK cascade.	gene_phenotype
70944	3	334171	7	NULL	NULL	0	NULL	statement 2	Process		occur in					Hog1 MAPK cascade	Process	osmostress signaling to 			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_273	10749922	Mpr1 is most homologous to the budding yeast Ypd1 protein, which transfers a phosphoryl group from the receiver domain of Sln1 to the Ssk1 response regulator in osmostress signaling to the Hog1 MAPK cascade.	gene_phenotype
70945	4	334171	7	NULL	NULL	0	NULL	Ypd1 protein	GP		carries out					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_273	10749922	Mpr1 is most homologous to the budding yeast Ypd1 protein, which transfers a phosphoryl group from the receiver domain of Sln1 to the Ssk1 response regulator in osmostress signaling to the Hog1 MAPK cascade.	gene_phenotype
70946	1	334172	7	NULL	NULL	0	NULL	Mpr1-Mcs4 pathway	Process		is highly					conserved	Process				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_278	10749922	Considering the highly conserved architecture of the Mpr1-Mcs4 pathway and the budding yeast Ypd1-Ssk1 pathway, it is surprising that Mpr1 and Mcs4 are involved in transmitting oxidative stress rather than osmostress signals to a SAPK cascade.	gene_phenotype
70947	2	334172	7	NULL	NULL	NULL	NULL	Ypd1-Ssk1 pathway	Process		is highly					conserved	Process				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_278	10749922	Considering the highly conserved architecture of the Mpr1-Mcs4 pathway and the budding yeast Ypd1-Ssk1 pathway, it is surprising that Mpr1 and Mcs4 are involved in transmitting oxidative stress rather than osmostress signals to a SAPK cascade.	gene_phenotype
70948	3	334172	7	NULL	NULL	0	NULL	Mpr1	GP		is involved in					oxidative stress	Process	transmitting 			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_278	10749922	Considering the highly conserved architecture of the Mpr1-Mcs4 pathway and the budding yeast Ypd1-Ssk1 pathway, it is surprising that Mpr1 and Mcs4 are involved in transmitting oxidative stress rather than osmostress signals to a SAPK cascade.	gene_phenotype
70949	4	334172	7	NULL	NULL	0	NULL	Mcs4	GP		is involved in					oxidative stress	Process	transmitting 			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_278	10749922	Considering the highly conserved architecture of the Mpr1-Mcs4 pathway and the budding yeast Ypd1-Ssk1 pathway, it is surprising that Mpr1 and Mcs4 are involved in transmitting oxidative stress rather than osmostress signals to a SAPK cascade.	gene_phenotype
70950	5	334172	7	NULL	NULL	0	NULL	Mpr1	GP		is not involved in					 osmostress signals 	Process	transmitting 			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_278	10749922	Considering the highly conserved architecture of the Mpr1-Mcs4 pathway and the budding yeast Ypd1-Ssk1 pathway, it is surprising that Mpr1 and Mcs4 are involved in transmitting oxidative stress rather than osmostress signals to a SAPK cascade.	gene_phenotype
70951	6	334172	7	NULL	NULL	0	NULL	Mcs4	GP		is not involved in					osmostress signaling	Process	transmitting 			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_278	10749922	Considering the highly conserved architecture of the Mpr1-Mcs4 pathway and the budding yeast Ypd1-Ssk1 pathway, it is surprising that Mpr1 and Mcs4 are involved in transmitting oxidative stress rather than osmostress signals to a SAPK cascade.	gene_phenotype
70952	7	334172	7	NULL	NULL	0	NULL	osmostress signals	Process		in response to					SAPK cascade	Process				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_278	10749922	Considering the highly conserved architecture of the Mpr1-Mcs4 pathway and the budding yeast Ypd1-Ssk1 pathway, it is surprising that Mpr1 and Mcs4 are involved in transmitting oxidative stress rather than osmostress signals to a SAPK cascade.	gene_phenotype
70953	1	334173	7	NULL	NULL	0	NULL	MPR1 gene	GP	expression of;;strain FH506	confers					AZC resistance	Process	S. cerevisiae strain			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_15_4249_s_206	10894734	Expression of the  MPR1 and  MPR2 genes isolated from strain FH506 conferred AZC resistance to other  S. cerevisiae strains but did not cause increases in proline content and cell viability after freezing of the host cells (data not shown).	gene_phenotype
70954	2	334173	7	NULL	NULL	0	NULL	MPR2 gene	GP	expression of;;strain FH506	confers					AZC resistance	Process	S. cerevisiae strain			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_15_4249_s_206	10894734	Expression of the  MPR1 and  MPR2 genes isolated from strain FH506 conferred AZC resistance to other  S. cerevisiae strains but did not cause increases in proline content and cell viability after freezing of the host cells (data not shown).	gene_phenotype
70955	3	334173	7	NULL	NULL	NULL	NULL	MPR1 gene	GP	expression of;;strain FH506	does not increase					proline content	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_15_4249_s_206	10894734	Expression of the  MPR1 and  MPR2 genes isolated from strain FH506 conferred AZC resistance to other  S. cerevisiae strains but did not cause increases in proline content and cell viability after freezing of the host cells (data not shown).	gene_phenotype
70956	4	334173	7	NULL	NULL	0	NULL	MPR2 gene	GP	expression of;;strain FH506	does not increase					proline content	AminoAcid				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_15_4249_s_206	10894734	Expression of the  MPR1 and  MPR2 genes isolated from strain FH506 conferred AZC resistance to other  S. cerevisiae strains but did not cause increases in proline content and cell viability after freezing of the host cells (data not shown).	gene_phenotype
70957	5	334173	7	NULL	NULL	0	NULL	MPR1 gene	GP	expression of;;strain FH506	does not increase					cell viability	Process				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_15_4249_s_206	10894734	Expression of the  MPR1 and  MPR2 genes isolated from strain FH506 conferred AZC resistance to other  S. cerevisiae strains but did not cause increases in proline content and cell viability after freezing of the host cells (data not shown).	gene_phenotype
70958	6	334173	7	NULL	NULL	0	NULL	MPR2 gene	GP	expression of;;strain FH506	does not increase					cell viability	Process				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_15_4249_s_206	10894734	Expression of the  MPR1 and  MPR2 genes isolated from strain FH506 conferred AZC resistance to other  S. cerevisiae strains but did not cause increases in proline content and cell viability after freezing of the host cells (data not shown).	gene_phenotype
70959	1	334176	7	NULL	NULL	0	NULL	oxidative stress	Process		activates					Spc1	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_5	10749922	Spc1 activation upon oxidative stress is severely impaired in the  deltampr1 mutant as well as in the  mpr1HQ strain, in which the putative phosphorylation site Mpr1-His221 is substituted with glutamine.	gene_phenotype
70960	2	334176	7	NULL	NULL	NULL	NULL	statement 1	Process		is  impaired in		severely			deltampr1	GP	mutant			NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_5	10749922	Spc1 activation upon oxidative stress is severely impaired in the  deltampr1 mutant as well as in the  mpr1HQ strain, in which the putative phosphorylation site Mpr1-His221 is substituted with glutamine.	gene_phenotype
70961	3	334176	7	NULL	NULL	NULL	NULL	statement 1	Process		is impaired in		severely			mpr1HQ strain	Organism				NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_5	10749922	Spc1 activation upon oxidative stress is severely impaired in the  deltampr1 mutant as well as in the  mpr1HQ strain, in which the putative phosphorylation site Mpr1-His221 is substituted with glutamine.	gene_phenotype
70962	4	334176	7	NULL	NULL	0	NULL	mpr1HQ strain	Organism		is substituted with			putative phosphorylation site Mpr1-His221		mpr1HQ strain	Organism		putative phosphorylation site Mpr1-Gln221		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_11_4_1169_s_5	10749922	Spc1 activation upon oxidative stress is severely impaired in the  deltampr1 mutant as well as in the  mpr1HQ strain, in which the putative phosphorylation site Mpr1-His221 is substituted with glutamine.	gene_phenotype
70963	1	334178	7	NULL	NULL	0	NULL	RPN11	GP		complements					mpr1-1 	GP	temperature-sensitive growth of			NULL		0	NULL	NULL	NULL	gw60_science_298_5593_611_s_81	12183636	Plasmid-borne  RPN11 but not  rpn11AXA complemented the temperature-sensitive growth of  mpr1-1 ( Fig. 2C).	gene_phenotype
70964	2	334178	7	NULL	NULL	0	NULL	rpn11AXA	GP		does not complement					mpr1-1 	GP	temperature-sensitive growth of			NULL		0	NULL	NULL	NULL	gw60_science_298_5593_611_s_81	12183636	Plasmid-borne  RPN11 but not  rpn11AXA complemented the temperature-sensitive growth of  mpr1-1 ( Fig. 2C).	gene_phenotype
70965	1	334179	7	NULL	NULL	0	NULL	ry 	GP	mutation of	restores					mpr1-1	GP	defect of;;mutant			NULL		0	NULL	NULL	NULL	gw60_gene_286_1_43_s_138	11943459	The  ry mutation which restores a defect of the  mpr1-1 mutant indicates the existence of an additional factor interacting with Rpn11 and involved in the maintenance of the mitochondrial morphology.	gene_phenotype
70966	1	334180	7	NULL	NULL	0	NULL	mpr1-1	GP	effects of mutation on	is restored in					 Wm-ru-ry	GP	triple mutant			NULL		0	NULL	NULL	NULL	gw60_gene_286_1_43_s_136	11943459	The effects of  mpr1-1 mutation on mitochondrial morphology are only restored in the Wm-ru-ry triple mutant which was isolated from Wm-ru as a spontaneous revertant which grows on non-fermentable carbon source at 36 degrees C.	gene_phenotype
70967	1	334181	7	NULL	NULL	0	NULL	mpr1-1 cells	Cell		displays					aberrant morphology	Process				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_9_10_2917_s_170	9763452	In this condition,  mpr1-1 cells exhibited an aberrant morphology characterized by elongated daughter cells unable to perform a further division, whereas the nucleus was mislocalized and often only present in the first bud (Figure  4E).	gene_phenotype
70968	2	334181	7	NULL	NULL	0	NULL	aberrant morphology	Process		characterized by					elongated daughter cells	Cell				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_9_10_2917_s_170	9763452	In this condition,  mpr1-1 cells exhibited an aberrant morphology characterized by elongated daughter cells unable to perform a further division, whereas the nucleus was mislocalized and often only present in the first bud (Figure  4E).	gene_phenotype
70969	3	334181	7	NULL	NULL	0	NULL	elongated daughter cells	Cell		does not undergo					division	Process				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_9_10_2917_s_170	9763452	In this condition,  mpr1-1 cells exhibited an aberrant morphology characterized by elongated daughter cells unable to perform a further division, whereas the nucleus was mislocalized and often only present in the first bud (Figure  4E).	gene_phenotype
70970	4	334181	7	NULL	NULL	0	NULL	elongated daughter cells	cell		shows					mislocalized nucleus	CellComponent				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_9_10_2917_s_170	9763452	In this condition,  mpr1-1 cells exhibited an aberrant morphology characterized by elongated daughter cells unable to perform a further division, whereas the nucleus was mislocalized and often only present in the first bud (Figure  4E).	gene_phenotype
70971	1	334182	7	NULL	NULL	0	NULL	 punctate mitochondrial morphology 	GP		is observed in					 mpr1-1	GP	mutant			NULL		0	NULL	NULL	NULL	gw60_molbiolcell_9_10_2917_s_276	9763452	The punctate mitochondrial morphology we observe in the  mpr1-1 mutant growing on rich medium containing glucose has also been observed in the  yme1 mutant altered in a mitochondrial protease.	gene_phenotype
70972	2	334182	7	NULL	NULL	0	NULL	yme1	GP	mutant	altered in					mitochondrial protease	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_9_10_2917_s_276	9763452	The punctate mitochondrial morphology we observe in the  mpr1-1 mutant growing on rich medium containing glucose has also been observed in the  yme1 mutant altered in a mitochondrial protease.	gene_phenotype
70973	3	334182	7	NULL	NULL	0	NULL	punctate mitochondrial morphology	Process		is observed in					statement 2	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_9_10_2917_s_276	9763452	The punctate mitochondrial morphology we observe in the  mpr1-1 mutant growing on rich medium containing glucose has also been observed in the  yme1 mutant altered in a mitochondrial protease.	gene_phenotype
70974	1	334183	7	NULL	NULL	0	NULL	mpr1-1	GP	mutant	reveals					mitosis	Process	defect in exit from			NULL		0	NULL	NULL	NULL	gw60_gene_286_1_43_s_81	11943459	Microscopic observation of the  mpr1-1 mutant strain after DAPI staining had previously revealed a defect in the exit from mitosis, with large buds during growth at 24 degrees C and aberrant bud morphology when cells were shifted at the non-permissive temperature.	gene_phenotype
70975	1	334184	7	NULL	NULL	NULL	NULL	DNA	NucleicAcid	increase in	is not restricted to					nuclear DNA	NucleicAcid	increase of			NULL	 [ rho+] mpr1-1 strain	NULL	NULL	NULL	NULL	gw60_molbiolcell_9_10_2917_s_199	9763452	In other words, the increase in DNA content per cell is not restricted to an increase of nuclear DNA but reaches higher values in the [ rho+]  mpr1-1 strain than in the [ rho degrees ] derivative, suggesting an important contribution of mitochondrial DNA to the aberrant flow cytometry profile.	gene_phenotype
70977	1	334185	7	NULL	NULL	NULL	NULL	mpr1-1	GP	frameshift in 	leads to			RPN11		temperature-sensitive growth	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_298_5593_611_s_80	12183636	To facilitate further phenotypic characterization of the  AXA mutant, we used  mpr1-1, which contains a frameshift in  RPN11 that leads to temperature-sensitive growth and expression of a prematurely terminated Rpn11mpr1-1 protein (285 versus 306 amino acids for wild type) ( 16).	gene_phenotype
70978	2	334185	7	NULL	NULL	0	NULL	mpr1-1	GP	frameshift in 	leads to			RPN11		Rpn11mpr1-1 protein	GP	expression of;;prematurely terminated 			NULL		0	NULL	NULL	NULL	gw60_science_298_5593_611_s_80	12183636	To facilitate further phenotypic characterization of the  AXA mutant, we used  mpr1-1, which contains a frameshift in  RPN11 that leads to temperature-sensitive growth and expression of a prematurely terminated Rpn11mpr1-1 protein (285 versus 306 amino acids for wild type) ( 16).	gene_phenotype
70979	1	334187	7	NULL	NULL	0	NULL	scR1 	GP	Nuclear export of	is mediated by					Xpo1p	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_8	11352936	Nuclear export of scR1 is mediated by the nuclear export signal receptor Xpo1p, is distinct from mRNA transport, and requires, as evidenced by the nucleolar accumulation of scR1 in a  dis3/rrp44 exosome component mutant, an intact scR1 3' end.	gene_phenotype
70980	2	334187	7	NULL	NULL	0	NULL	Xpo1p	GP		is a type of					nuclear export signal receptor	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_8	11352936	Nuclear export of scR1 is mediated by the nuclear export signal receptor Xpo1p, is distinct from mRNA transport, and requires, as evidenced by the nucleolar accumulation of scR1 in a  dis3/rrp44 exosome component mutant, an intact scR1 3' end.	gene_phenotype
70981	3	334187	7	NULL	NULL	0	NULL	statement 1	Process		is distinct from					mRNA 	NucleicAcid	transport of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_8	11352936	Nuclear export of scR1 is mediated by the nuclear export signal receptor Xpo1p, is distinct from mRNA transport, and requires, as evidenced by the nucleolar accumulation of scR1 in a  dis3/rrp44 exosome component mutant, an intact scR1 3' end.	gene_phenotype
70982	4	334187	7	NULL	NULL	0	NULL	statement 1	Process		requires					scR1	GP	nucleolar accumulation of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_8	11352936	Nuclear export of scR1 is mediated by the nuclear export signal receptor Xpo1p, is distinct from mRNA transport, and requires, as evidenced by the nucleolar accumulation of scR1 in a  dis3/rrp44 exosome component mutant, an intact scR1 3' end.	gene_phenotype
70983	5	334187	7	NULL	NULL	0	NULL	statement 4	Process		occur in a					dis3/rrp44 exosome component mutant	CellComponent				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_8	11352936	Nuclear export of scR1 is mediated by the nuclear export signal receptor Xpo1p, is distinct from mRNA transport, and requires, as evidenced by the nucleolar accumulation of scR1 in a  dis3/rrp44 exosome component mutant, an intact scR1 3' end.	gene_phenotype
70984	6	334187	7	NULL	NULL	0	NULL	statement 1	Process		requires					scR1	GP		intact 3' end		NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_8	11352936	Nuclear export of scR1 is mediated by the nuclear export signal receptor Xpo1p, is distinct from mRNA transport, and requires, as evidenced by the nucleolar accumulation of scR1 in a  dis3/rrp44 exosome component mutant, an intact scR1 3' end.	gene_phenotype
70985	1	334189	7	NULL	NULL	0	NULL	Ran cycle	Process	intact	is required for					scR1	GP	nuclear export of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_170	11352936	These data show that an intact Ran cycle is required for scR1 nuclear export.	gene_phenotype
70986	1	334190	7	NULL	NULL	NULL	NULL	exportin	GP		be involved in		might			scR1	GP	nuclear export of			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_172	11352936	Alternatively, (an) exportin(s) might be involved in scR1 nuclear export.	gene_phenotype
70987	1	334191	7	NULL	NULL	0	NULL	scR1	GP		exported to					nucleus	CellComponent				NULL	LMB-sensitive strain	0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_201	11352936	Therefore, we analyzed nuclear export of scR1 in the LMB-sensitive strain.	gene_phenotype
70988	1	334192	7	NULL	NULL	0	NULL	Nucleoporins	CellComponent	subset of	is involved in					scR1	GP	nuclear export of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_266	11352936	A Subset of Nucleoporins Is Involved in scR1 Nuclear Export   The finding that Nsp1p is required for scR1 nuclear export prompted us to investigate the requirement of NPC components in this process.	gene_phenotype
70989	2	334192	7	NULL	NULL	0	NULL	Nsp1p	GP		is required for					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_266	11352936	A Subset of Nucleoporins Is Involved in scR1 Nuclear Export   The finding that Nsp1p is required for scR1 nuclear export prompted us to investigate the requirement of NPC components in this process.	gene_phenotype
70990	1	334193	7	NULL	NULL	NULL	NULL	scR1	GP		is required for			intact 3' end		scR1	GP	nuclear export of			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_328	11352936	The correlation between this 3' end shortening and nucleolar accumulation of scR1 in the  rrp44-1 mutant cells suggests that an intact 3' end is required for scR1 nuclear export.	gene_phenotype
70991	2	334193	7	NULL	NULL	0	NULL	scR1	GP		accumulates in					nucleolus	Cell				NULL	 rrp44-1 mutant cells	0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_328	11352936	The correlation between this 3' end shortening and nucleolar accumulation of scR1 in the  rrp44-1 mutant cells suggests that an intact 3' end is required for scR1 nuclear export.	gene_phenotype
70992	3	334193	7	NULL	NULL	0	NULL	statement 2	Process		suggests					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_328	11352936	The correlation between this 3' end shortening and nucleolar accumulation of scR1 in the  rrp44-1 mutant cells suggests that an intact 3' end is required for scR1 nuclear export.	gene_phenotype
70993	1	334194	7	NULL	NULL	NULL	NULL	flies 	Organism	heterozygous deletions	viable with					Scr1	GP				NULL		NULL	NULL	NULL	NULL	gw60_genetics_161_2_733_s_115	12072469	We observed similar results with the hypomorphic mutation  Scr1, but because the viability of flies heterozygous for the deletions was much greater with  Scr1 than with  Scr4, we were able to examine more males.	gene_phenotype
70994	2	334194	7	NULL	NULL	NULL	NULL	flies	Organism	 heterozygous deletions	viable with					Scr4	GP				NULL		NULL	NULL	NULL	NULL	gw60_genetics_161_2_733_s_115	12072469	We observed similar results with the hypomorphic mutation  Scr1, but because the viability of flies heterozygous for the deletions was much greater with  Scr1 than with  Scr4, we were able to examine more males.	gene_phenotype
70995	3	334194	7	NULL	NULL	0	NULL	statement 1	Process	viability of	is greater than					statement 2	Process	viability of			NULL		0	NULL	NULL	NULL	gw60_genetics_161_2_733_s_115	12072469	We observed similar results with the hypomorphic mutation  Scr1, but because the viability of flies heterozygous for the deletions was much greater with  Scr1 than with  Scr4, we were able to examine more males.	gene_phenotype
70996	1	334195	7	NULL	NULL	0	NULL	Core SRP Proteins 	GP		concentrate in					Nucleolus	CellComponent				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_134	11352936	The Core SRP Proteins Concentrate in the Nucleolus   The requirement of the four SRP core proteins for the export of scR1 into the cytoplasm suggests that these proteins assemble with scR1 inside the nucleus to form a transport-competent particle.	gene_phenotype
70997	2	334195	7	NULL	NULL	0	NULL	 scR1	GP		exported to					cytoplasm	CellComponent				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_134	11352936	The Core SRP Proteins Concentrate in the Nucleolus   The requirement of the four SRP core proteins for the export of scR1 into the cytoplasm suggests that these proteins assemble with scR1 inside the nucleus to form a transport-competent particle.	gene_phenotype
70998	3	334195	7	NULL	NULL	0	NULL	four SRP core proteins	GP		required for					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_134	11352936	The Core SRP Proteins Concentrate in the Nucleolus   The requirement of the four SRP core proteins for the export of scR1 into the cytoplasm suggests that these proteins assemble with scR1 inside the nucleus to form a transport-competent particle.	gene_phenotype
70999	4	334195	7	NULL	NULL	0	NULL	four SRP core proteins	GP		assemble with					scR1	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_134	11352936	The Core SRP Proteins Concentrate in the Nucleolus   The requirement of the four SRP core proteins for the export of scR1 into the cytoplasm suggests that these proteins assemble with scR1 inside the nucleus to form a transport-competent particle.	gene_phenotype
71000	5	334195	7	NULL	NULL	0	NULL	statement 4	Process		occur in					nucleus	CellComponent				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_134	11352936	The Core SRP Proteins Concentrate in the Nucleolus   The requirement of the four SRP core proteins for the export of scR1 into the cytoplasm suggests that these proteins assemble with scR1 inside the nucleus to form a transport-competent particle.	gene_phenotype
71001	6	334195	7	NULL	NULL	0	NULL	statement 5	Process		form					 transport-competent particle	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_134	11352936	The Core SRP Proteins Concentrate in the Nucleolus   The requirement of the four SRP core proteins for the export of scR1 into the cytoplasm suggests that these proteins assemble with scR1 inside the nucleus to form a transport-competent particle.	gene_phenotype
71002	7	334195	7	NULL	NULL	0	NULL	statement 3	Process		suggests					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_134	11352936	The Core SRP Proteins Concentrate in the Nucleolus   The requirement of the four SRP core proteins for the export of scR1 into the cytoplasm suggests that these proteins assemble with scR1 inside the nucleus to form a transport-competent particle.	gene_phenotype
71003	1	334196	7	NULL	NULL	0	NULL	scR1	GP		localizes in		normally			los1- mutant cells	Cell				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_174	11352936	In the  los1-,  cse1-1, and  msn5- mutant cells, the localization of scR1 was normal and indistinguishable from that in wild-type cells, suggesting that the corresponding proteins are not involved in the nuclear export of scR1 (data not shown).	gene_phenotype
71004	2	334196	7	NULL	NULL	0	NULL	scR1	GP		localizes in		normally			cse1-1 mutant cells	Cell				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_174	11352936	In the  los1-,  cse1-1, and  msn5- mutant cells, the localization of scR1 was normal and indistinguishable from that in wild-type cells, suggesting that the corresponding proteins are not involved in the nuclear export of scR1 (data not shown).	gene_phenotype
71005	3	334196	7	NULL	NULL	NULL	NULL	scR1	GP		localizes in		normally			msn5- mutant cells	Cell				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_174	11352936	In the  los1-,  cse1-1, and  msn5- mutant cells, the localization of scR1 was normal and indistinguishable from that in wild-type cells, suggesting that the corresponding proteins are not involved in the nuclear export of scR1 (data not shown).	gene_phenotype
71006	4	334196	7	NULL	NULL	0	NULL	 los1	GP		is not involved in					scR1	GP	nuclear export of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_174	11352936	In the  los1-,  cse1-1, and  msn5- mutant cells, the localization of scR1 was normal and indistinguishable from that in wild-type cells, suggesting that the corresponding proteins are not involved in the nuclear export of scR1 (data not shown).	gene_phenotype
71007	5	334196	7	NULL	NULL	0	NULL	cse1-1	GP		is not involved in					scR1	GP	nuclear export of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_174	11352936	In the  los1-,  cse1-1, and  msn5- mutant cells, the localization of scR1 was normal and indistinguishable from that in wild-type cells, suggesting that the corresponding proteins are not involved in the nuclear export of scR1 (data not shown).	gene_phenotype
71008	6	334196	7	NULL	NULL	0	NULL	msn5	GP		is not involved in					scR1	GP	nuclear export of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_174	11352936	In the  los1-,  cse1-1, and  msn5- mutant cells, the localization of scR1 was normal and indistinguishable from that in wild-type cells, suggesting that the corresponding proteins are not involved in the nuclear export of scR1 (data not shown).	gene_phenotype
71009	7	334196	7	NULL	NULL	0	NULL	statement 1	Process		is indistinguishable from					wild-type cells	Cell				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_174	11352936	In the  los1-,  cse1-1, and  msn5- mutant cells, the localization of scR1 was normal and indistinguishable from that in wild-type cells, suggesting that the corresponding proteins are not involved in the nuclear export of scR1 (data not shown).	gene_phenotype
71010	8	334196	7	NULL	NULL	0	NULL	statement 2	Process		is indistinguishable from					wild-type cells	Cell				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_174	11352936	In the  los1-,  cse1-1, and  msn5- mutant cells, the localization of scR1 was normal and indistinguishable from that in wild-type cells, suggesting that the corresponding proteins are not involved in the nuclear export of scR1 (data not shown).	gene_phenotype
71011	9	334196	7	NULL	NULL	0	NULL	statement 3	Process		is indistinguishable from					wild-type cells	Cell				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_174	11352936	In the  los1-,  cse1-1, and  msn5- mutant cells, the localization of scR1 was normal and indistinguishable from that in wild-type cells, suggesting that the corresponding proteins are not involved in the nuclear export of scR1 (data not shown).	gene_phenotype
71012	10	334196	7	NULL	NULL	0	NULL	statement 1	Process		suggest					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_174	11352936	In the  los1-,  cse1-1, and  msn5- mutant cells, the localization of scR1 was normal and indistinguishable from that in wild-type cells, suggesting that the corresponding proteins are not involved in the nuclear export of scR1 (data not shown).	gene_phenotype
71013	11	334196	7	NULL	NULL	0	NULL	statement 2	Process		suggest					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_174	11352936	In the  los1-,  cse1-1, and  msn5- mutant cells, the localization of scR1 was normal and indistinguishable from that in wild-type cells, suggesting that the corresponding proteins are not involved in the nuclear export of scR1 (data not shown).	gene_phenotype
71014	12	334196	7	NULL	NULL	0	NULL	statement 3	Process		suggest					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_174	11352936	In the  los1-,  cse1-1, and  msn5- mutant cells, the localization of scR1 was normal and indistinguishable from that in wild-type cells, suggesting that the corresponding proteins are not involved in the nuclear export of scR1 (data not shown).	gene_phenotype
71015	1	334197	7	NULL	NULL	0	NULL	rrp44-1 cells	Cell	mutation in	does not affect					scR1	GP	overall stability of 			NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_241	11352936	Taken together, these data suggest that the mutation in the  rrp44-1 cells does not affect the overall stability of scR1, but leads to aberrant processing of scR1 3' ends, thus possibly rendering the RNA incompetent for nuclear export.	gene_phenotype
71016	2	334197	7	NULL	NULL	0	NULL	rrp44-1 cells	Cell	mutation in	leads to					scR1	GP	aberrant processing of	3' end		NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_241	11352936	Taken together, these data suggest that the mutation in the  rrp44-1 cells does not affect the overall stability of scR1, but leads to aberrant processing of scR1 3' ends, thus possibly rendering the RNA incompetent for nuclear export.	gene_phenotype
71017	3	334197	7	NULL	NULL	NULL	NULL	statement 2	Process		renders		possibly			RNA	NucleicAcid	incompetent 			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_241	11352936	Taken together, these data suggest that the mutation in the  rrp44-1 cells does not affect the overall stability of scR1, but leads to aberrant processing of scR1 3' ends, thus possibly rendering the RNA incompetent for nuclear export.	gene_phenotype
71018	4	334197	7	NULL	NULL	NULL	NULL	RNA	NucleicAcid		required for					scR1	Process	nuclear export of			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_241	11352936	Taken together, these data suggest that the mutation in the  rrp44-1 cells does not affect the overall stability of scR1, but leads to aberrant processing of scR1 3' ends, thus possibly rendering the RNA incompetent for nuclear export.	gene_phenotype
71019	1	334198	7	NULL	NULL	0	NULL	Nsp1p 	GP		is required for					SRP-RNA	GP	nuclear export of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_242	11352936	The Essential Nucleoporin Nsp1p Is Required for SRP-RNA Nuclear Export   o find other factors involved in scR1 nuclear export, we started screening a collection of random yeast  ts mutants using the scR1 FISH assay.	gene_phenotype
71020	2	334198	7	NULL	NULL	0	NULL	Nsp1p	GP		is a type of					Nucleoporin	CellComponent	essential			NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_242	11352936	The Essential Nucleoporin Nsp1p Is Required for SRP-RNA Nuclear Export   o find other factors involved in scR1 nuclear export, we started screening a collection of random yeast  ts mutants using the scR1 FISH assay.	gene_phenotype
71021	1	334199	7	NULL	NULL	0	NULL	sCCPH	GP		acts as					Factor I cofactor	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_184	16760474	Factor I cofactor activity of sCCPH, VCP, factor H ( fH), and sCR1 for complement proteins C3b and C4b.	gene_phenotype
71022	2	334199	7	NULL	NULL	0	NULL	VCP	GP		acts as					Factor I cofactor	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_184	16760474	Factor I cofactor activity of sCCPH, VCP, factor H ( fH), and sCR1 for complement proteins C3b and C4b.	gene_phenotype
71023	3	334199	7	NULL	NULL	0	NULL	factor H 	GP		acts as					Factor I cofactor	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_184	16760474	Factor I cofactor activity of sCCPH, VCP, factor H ( fH), and sCR1 for complement proteins C3b and C4b.	gene_phenotype
71024	4	334199	7	NULL	NULL	NULL	NULL	sCR1	GP		acts as					Factor I cofactor	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_184	16760474	Factor I cofactor activity of sCCPH, VCP, factor H ( fH), and sCR1 for complement proteins C3b and C4b.	gene_phenotype
71025	5	334199	7	NULL	NULL	0	NULL	fH	GP		is					factor H	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_184	16760474	Factor I cofactor activity of sCCPH, VCP, factor H ( fH), and sCR1 for complement proteins C3b and C4b.	gene_phenotype
71026	6	334199	7	NULL	NULL	NULL	NULL	statement 1	GP		cofactor for					C3b	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_184	16760474	Factor I cofactor activity of sCCPH, VCP, factor H ( fH), and sCR1 for complement proteins C3b and C4b.	gene_phenotype
71027	7	334199	7	NULL	NULL	NULL	NULL	statement 1	GP		cofactor for					C4b	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_184	16760474	Factor I cofactor activity of sCCPH, VCP, factor H ( fH), and sCR1 for complement proteins C3b and C4b.	gene_phenotype
71028	8	334199	7	NULL	NULL	0	NULL	statement 2	GP		cofactor for					C3b	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_184	16760474	Factor I cofactor activity of sCCPH, VCP, factor H ( fH), and sCR1 for complement proteins C3b and C4b.	gene_phenotype
71029	9	334199	7	NULL	NULL	0	NULL	statement 2	GP		cofactor for					C4b	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_184	16760474	Factor I cofactor activity of sCCPH, VCP, factor H ( fH), and sCR1 for complement proteins C3b and C4b.	gene_phenotype
71030	10	334199	7	NULL	NULL	0	NULL	statement 3	GP		cofactor for					C3b	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_184	16760474	Factor I cofactor activity of sCCPH, VCP, factor H ( fH), and sCR1 for complement proteins C3b and C4b.	gene_phenotype
71031	11	334199	7	NULL	NULL	0	NULL	statement 3	GP		cofactor for					C4b	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_184	16760474	Factor I cofactor activity of sCCPH, VCP, factor H ( fH), and sCR1 for complement proteins C3b and C4b.	gene_phenotype
71032	12	334199	7	NULL	NULL	0	NULL	statement 4	GP		cofactor for					C3b	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_184	16760474	Factor I cofactor activity of sCCPH, VCP, factor H ( fH), and sCR1 for complement proteins C3b and C4b.	gene_phenotype
71033	13	334199	7	NULL	NULL	0	NULL	statement 4	GP		cofactor for					C4b	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_184	16760474	Factor I cofactor activity of sCCPH, VCP, factor H ( fH), and sCR1 for complement proteins C3b and C4b.	gene_phenotype
71034	14	334199	7	NULL	NULL	0	NULL	C3b	GP		is a type of					complement protein	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_184	16760474	Factor I cofactor activity of sCCPH, VCP, factor H ( fH), and sCR1 for complement proteins C3b and C4b.	gene_phenotype
71035	15	334199	7	NULL	NULL	0	NULL	C4b	GP		is a type of					complement protein	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_184	16760474	Factor I cofactor activity of sCCPH, VCP, factor H ( fH), and sCR1 for complement proteins C3b and C4b.	gene_phenotype
71036	1	334200	7	NULL	NULL	0	NULL	 sCCPH	GP		acts as					Factor I cofactor	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_193	16760474	Time course of factor I cofactor activity of sCCPH, VCP, factor H ( fH), and sCR1 for complement protein C3b.	gene_phenotype
71037	2	334200	7	NULL	NULL	0	NULL	VCP	GP		acts as					Factor I cofactor	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_193	16760474	Time course of factor I cofactor activity of sCCPH, VCP, factor H ( fH), and sCR1 for complement protein C3b.	gene_phenotype
71038	3	334200	7	NULL	NULL	0	NULL	fH	GP		acts as					Factor I cofactor	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_193	16760474	Time course of factor I cofactor activity of sCCPH, VCP, factor H ( fH), and sCR1 for complement protein C3b.	gene_phenotype
71039	4	334200	7	NULL	NULL	0	NULL	sCR1	GP		acts as					Factor I cofactor	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_193	16760474	Time course of factor I cofactor activity of sCCPH, VCP, factor H ( fH), and sCR1 for complement protein C3b.	gene_phenotype
71041	5	334200	7	NULL	NULL	0	NULL	statement 1	GP		cofactor for					C3b	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_193	16760474	Time course of factor I cofactor activity of sCCPH, VCP, factor H ( fH), and sCR1 for complement protein C3b.	gene_phenotype
71042	6	334200	7	NULL	NULL	0	NULL	statement 2	GP		cofactor for					C3b	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_193	16760474	Time course of factor I cofactor activity of sCCPH, VCP, factor H ( fH), and sCR1 for complement protein C3b.	gene_phenotype
71044	7	334200	7	NULL	NULL	0	NULL	statement 3	GP		cofactor for					C3b	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_193	16760474	Time course of factor I cofactor activity of sCCPH, VCP, factor H ( fH), and sCR1 for complement protein C3b.	gene_phenotype
71046	8	334200	7	NULL	NULL	0	NULL	statement 4	GP		cofactor for					C3b	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_193	16760474	Time course of factor I cofactor activity of sCCPH, VCP, factor H ( fH), and sCR1 for complement protein C3b.	gene_phenotype
71049	9	334200	7	NULL	NULL	0	NULL	C3b	GP		is a type of					complement protein	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_193	16760474	Time course of factor I cofactor activity of sCCPH, VCP, factor H ( fH), and sCR1 for complement protein C3b.	gene_phenotype
71051	10	334200	7	NULL	NULL	0	NULL	fH	GP		is					factor H	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_193	16760474	Time course of factor I cofactor activity of sCCPH, VCP, factor H ( fH), and sCR1 for complement protein C3b.	gene_phenotype
71072	1	334201	7	NULL	NULL	0	NULL	sCCPH	GP		acts as					Factor I cofactor	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_227	16760474	Time course of factor I cofactor activity of sCCPH, VCP, and sCR1 for complement protein  C4b.	gene_phenotype
71073	2	334201	7	NULL	NULL	0	NULL	VCP	GP		acts as					Factor I cofactor	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_227	16760474	Time course of factor I cofactor activity of sCCPH, VCP, and sCR1 for complement protein  C4b.	gene_phenotype
71074	3	334201	7	NULL	NULL	0	NULL	sCR1	GP		acts as					Factor I cofactor	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_227	16760474	Time course of factor I cofactor activity of sCCPH, VCP, and sCR1 for complement protein  C4b.	gene_phenotype
71075	4	334201	7	NULL	NULL	0	NULL	statement 1	GP		cofactor for					C4b	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_227	16760474	Time course of factor I cofactor activity of sCCPH, VCP, and sCR1 for complement protein  C4b.	gene_phenotype
71076	5	334201	7	NULL	NULL	0	NULL	statement 2	GP		cofactor for					C4b	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_227	16760474	Time course of factor I cofactor activity of sCCPH, VCP, and sCR1 for complement protein  C4b.	gene_phenotype
71077	6	334201	7	NULL	NULL	0	NULL	statement 3	GP		cofactor for					C4b	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_227	16760474	Time course of factor I cofactor activity of sCCPH, VCP, and sCR1 for complement protein  C4b.	gene_phenotype
71078	7	334201	7	NULL	NULL	0	NULL	C4b	GP		is a type of					complement protein	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_227	16760474	Time course of factor I cofactor activity of sCCPH, VCP, and sCR1 for complement protein  C4b.	gene_phenotype
71086	1	334203	7	NULL	NULL	0	NULL	scR1	GP	export pathway of	is identical to					mRNA	NucleicAcid	export pathway of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_188	11352936	(A)+ RNA nuclear accumulation, or even reflects the use of identical export pathways for both scR1 and mRNA.	gene_phenotype
71090	1	334204	7	NULL	NULL	0	NULL	scR1		nuclear accumulation	is not consequence of					mRNA	NucleicAcid	export defect of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_192	11352936	(A)+ RNA, suggesting that the scR1 nuclear accumulation was not simply a consequence of the export defect for mRNA (data not shown).	gene_phenotype
71091	1	334205	7	NULL	NULL	0	NULL	mRNA	NucleicAcid	nuclear export mechanism of	is distinct from					scR1	GP	nuclear export mechanism of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_195	11352936	This, and the data presented below, strongly argue for distinct nuclear export mechanisms for mRNA and scR1.	gene_phenotype
71092	1	334206	7	NULL	NULL	0	NULL	scR1	GP	nuclear export of	involves		directly			Xpo1p	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_205	11352936	We conclude that nuclear export of scR1 directly involves the NES-export receptor Xpo1p and does not overlap with the mRNA export pathway.	gene_phenotype
71093	2	334206	7	NULL	NULL	0	NULL	Xpo1p	GP		is a type of					NES-export receptor	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_205	11352936	We conclude that nuclear export of scR1 directly involves the NES-export receptor Xpo1p and does not overlap with the mRNA export pathway.	gene_phenotype
71094	3	334206	7	NULL	NULL	0	NULL	statement 1	Process		does not overlap with					mRNA	NucleicAcid	export pathway of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_205	11352936	We conclude that nuclear export of scR1 directly involves the NES-export receptor Xpo1p and does not overlap with the mRNA export pathway.	gene_phenotype
71095	1	334208	7	NULL	NULL	0	NULL	 scR1	GP	strong nuclear export defect	present in					nup159 cells	Cell	mutant;;rat			NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_357	11352936	(A)+ RNA in the  srx1-1 cells at the restrictive temperature, as well as the strong scR1 nuclear export defect present in  nup159 ( rat7) mutant cells.	gene_phenotype
71096	1	334210	7	NULL	NULL	0	NULL	 sCCPH	GP		cofactor for					C4b	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_177	16760474	The cofactor activity of sCCPH for C4b was similar to VCP and sCR1, and like these proteins it also supported the cleavages at both the sites and led to generation of C4c and C4d.	gene_phenotype
71097	2	334210	7	NULL	NULL	0	NULL	VCP	GP		cofactor for					C4b	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_177	16760474	The cofactor activity of sCCPH for C4b was similar to VCP and sCR1, and like these proteins it also supported the cleavages at both the sites and led to generation of C4c and C4d.	gene_phenotype
71098	3	334210	7	NULL	NULL	0	NULL	sCR1	GP		cofactor for					C4b	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_177	16760474	The cofactor activity of sCCPH for C4b was similar to VCP and sCR1, and like these proteins it also supported the cleavages at both the sites and led to generation of C4c and C4d.	gene_phenotype
71099	4	334210	7	NULL	NULL	0	NULL	statement 1	Process		is similar to					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_177	16760474	The cofactor activity of sCCPH for C4b was similar to VCP and sCR1, and like these proteins it also supported the cleavages at both the sites and led to generation of C4c and C4d.	gene_phenotype
71100	5	334210	7	NULL	NULL	0	NULL	statement 1	Process		is similar to					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_177	16760474	The cofactor activity of sCCPH for C4b was similar to VCP and sCR1, and like these proteins it also supported the cleavages at both the sites and led to generation of C4c and C4d.	gene_phenotype
71101	6	334210	7	NULL	NULL	0	NULL	C4b	GP		cleaves to					C4c	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_177	16760474	The cofactor activity of sCCPH for C4b was similar to VCP and sCR1, and like these proteins it also supported the cleavages at both the sites and led to generation of C4c and C4d.	gene_phenotype
71102	7	334210	7	NULL	NULL	0	NULL	C4b	GP		cleaves to					C4d	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_177	16760474	The cofactor activity of sCCPH for C4b was similar to VCP and sCR1, and like these proteins it also supported the cleavages at both the sites and led to generation of C4c and C4d.	gene_phenotype
71103	8	334210	7	NULL	NULL	0	NULL	statement 6	Process		occur along with					statement 7	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_177	16760474	The cofactor activity of sCCPH for C4b was similar to VCP and sCR1, and like these proteins it also supported the cleavages at both the sites and led to generation of C4c and C4d.	gene_phenotype
71104	9	334210	7	NULL	NULL	0	NULL	sCCPH 	GP		supports 					statement 8	Process	cleavage of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_32_23119_s_177	16760474	The cofactor activity of sCCPH for C4b was similar to VCP and sCR1, and like these proteins it also supported the cleavages at both the sites and led to generation of C4c and C4d.	gene_phenotype
71105	1	334211	7	NULL	NULL	0	NULL	 anti-human CD46 mAb	GP		is specific for								SCR1 domain		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_28_25964_s_89	12724329	The cell mixture was lysed and subjected to  immunoprecipitation with an anti-human CD46 mAb (J4 - 48); this mAb is  specific for the SCR1 domain, which is dispensable for HHV-6 fusion  ( ,   ).	gene_phenotype
71106	2	334211	7	NULL	NULL	0	NULL				dispensable for			SCR1 domain		HHV-6 fusion	Organism				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_28_25964_s_89	12724329	The cell mixture was lysed and subjected to  immunoprecipitation with an anti-human CD46 mAb (J4 - 48); this mAb is  specific for the SCR1 domain, which is dispensable for HHV-6 fusion  ( ,   ).	gene_phenotype
71126	1	334213	7	NULL	NULL	0	NULL	 Xpo1p 	GP		is involved in					scR1 	GP	nuclear export of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_345	11352936	The involvement of Xpo1p in scR1 nuclear export was also suggested in another report that appeared shortly before this manuscript was submitted ( Ciufo and Brown 2000   ).	gene_phenotype
71127	1	334214	7	NULL	NULL	0	NULL	SRP	GP	yeast	is assembled into					core particle	GP				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_20_1256_s_42	11069106	Here, we report that yeast SRP is assembled in the nucleus into a core particle containing Srp14p, 21p, 68 and 72p, and scR1, which is a nuclear-export substrate.	gene_phenotype
71128	2	334214	7	NULL	NULL	0	NULL	core particle	GP		contains					Srp14p	GP				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_20_1256_s_42	11069106	Here, we report that yeast SRP is assembled in the nucleus into a core particle containing Srp14p, 21p, 68 and 72p, and scR1, which is a nuclear-export substrate.	gene_phenotype
71129	3	334214	7	NULL	NULL	0	NULL	core particle	GP		contains					Srp21p	GP				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_20_1256_s_42	11069106	Here, we report that yeast SRP is assembled in the nucleus into a core particle containing Srp14p, 21p, 68 and 72p, and scR1, which is a nuclear-export substrate.	gene_phenotype
71130	4	334214	7	NULL	NULL	0	NULL	core particle	GP		contains					Srp68p	GP				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_20_1256_s_42	11069106	Here, we report that yeast SRP is assembled in the nucleus into a core particle containing Srp14p, 21p, 68 and 72p, and scR1, which is a nuclear-export substrate.	gene_phenotype
71131	5	334214	7	NULL	NULL	0	NULL	core particle	GP		contains					Srp72p	GP				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_20_1256_s_42	11069106	Here, we report that yeast SRP is assembled in the nucleus into a core particle containing Srp14p, 21p, 68 and 72p, and scR1, which is a nuclear-export substrate.	gene_phenotype
71132	6	334214	7	NULL	NULL	0	NULL	core particle	GP		contains					 scR1	GP				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_20_1256_s_42	11069106	Here, we report that yeast SRP is assembled in the nucleus into a core particle containing Srp14p, 21p, 68 and 72p, and scR1, which is a nuclear-export substrate.	gene_phenotype
71133	7	334214	7	NULL	NULL	0	NULL	scR1	GP		is a type of					nuclear-export substrate	GP				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_20_1256_s_42	11069106	Here, we report that yeast SRP is assembled in the nucleus into a core particle containing Srp14p, 21p, 68 and 72p, and scR1, which is a nuclear-export substrate.	gene_phenotype
71134	8	334214	7	NULL	NULL	0	NULL	statement 1	Process		is assembled in					nucleus	CellComponent				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_20_1256_s_42	11069106	Here, we report that yeast SRP is assembled in the nucleus into a core particle containing Srp14p, 21p, 68 and 72p, and scR1, which is a nuclear-export substrate.	gene_phenotype
71135	9	334214	7	NULL	NULL	NULL	NULL	statement 2	GP		occur along with					statement 3	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_20_1256_s_42	11069106	Here, we report that yeast SRP is assembled in the nucleus into a core particle containing Srp14p, 21p, 68 and 72p, and scR1, which is a nuclear-export substrate.	gene_phenotype
71136	10	334214	7	NULL	NULL	NULL	NULL	statement 2	GP		occur along with					statement 4	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_20_1256_s_42	11069106	Here, we report that yeast SRP is assembled in the nucleus into a core particle containing Srp14p, 21p, 68 and 72p, and scR1, which is a nuclear-export substrate.	gene_phenotype
71137	11	334214	7	NULL	NULL	0	NULL	statement 2	GP		occur along with					statement 5	GP				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_20_1256_s_42	11069106	Here, we report that yeast SRP is assembled in the nucleus into a core particle containing Srp14p, 21p, 68 and 72p, and scR1, which is a nuclear-export substrate.	gene_phenotype
71138	12	334214	7	NULL	NULL	0	NULL	statement 2	GP		occur along with					statement 6	GP				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_20_1256_s_42	11069106	Here, we report that yeast SRP is assembled in the nucleus into a core particle containing Srp14p, 21p, 68 and 72p, and scR1, which is a nuclear-export substrate.	gene_phenotype
71139	1	334215	7	NULL	NULL	0	NULL	SRP components	GP		localizes in					nucleus	CellComponent				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_20_1256_s_135	11069106	A final issue raised by nuclear localisation of SRP components was which, if any, of the known pathways of export are responsible for transporting scR1 and the imported proteins to the cytoplasm.	gene_phenotype
71140	1	334216	7	NULL	NULL	NULL	NULL	scR1	GP		is present throughout					sporulation	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_43_40505_s_236	12181322	It is noteworthy that scR1, which was known to undergo very little variation in various physiological situations, is also present at a constant level throughout sporulation and spore germination.	gene_phenotype
71141	2	334216	7	NULL	NULL	0	NULL	scR1	GP		is present throughout					spore germination	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_43_40505_s_236	12181322	It is noteworthy that scR1, which was known to undergo very little variation in various physiological situations, is also present at a constant level throughout sporulation and spore germination.	gene_phenotype
71142	1	334218	7	NULL	NULL	0	NULL	 SCR1 gene 	GP		is unaffected by					silencing	Process	changes in 			NULL		0	NULL	NULL	NULL	gw60_science_276_5318_1547_s_109	9171055	To examine this  possibility, we quantitated mRNA levels of  GAL4-SIR1 and  normalized them to those of the  SCR1 gene ( 19),  whose expression is unaffected by changes in silencing or the cell  cycle.	gene_phenotype
71143	2	334218	7	NULL	NULL	0	NULL	SCR1 gene	GP		is unaffected by					cell cycle	Process	changes in			NULL		0	NULL	NULL	NULL	gw60_science_276_5318_1547_s_109	9171055	To examine this  possibility, we quantitated mRNA levels of  GAL4-SIR1 and  normalized them to those of the  SCR1 gene ( 19),  whose expression is unaffected by changes in silencing or the cell  cycle.	gene_phenotype
71144	1	334219	7	NULL	NULL	0	NULL	SCR1	GP		encode					natural cycloheximide resistance	Process	Schwanniomyces occidentalis			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_eur-j-biochem_213_2_8477754_s_2	8477754	Two genes (SCR1 and SCR2) encoding natural cycloheximide resistance in  the budding yeast Schwanniomyces occidentalis have been cloned by expression  in Saccharomyces cerevisiae.	gene_phenotype
71145	2	334219	7	NULL	NULL	0	NULL	 SCR2	GP		encode					natural cycloheximide resistance	Process	Schwanniomyces occidentalis			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_eur-j-biochem_213_2_8477754_s_2	8477754	Two genes (SCR1 and SCR2) encoding natural cycloheximide resistance in  the budding yeast Schwanniomyces occidentalis have been cloned by expression  in Saccharomyces cerevisiae.	gene_phenotype
71146	3	334219	7	NULL	NULL	0	NULL	Schwanniomyces occidentalis	Organism		is a type of					budding yeast	Organism				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_eur-j-biochem_213_2_8477754_s_2	8477754	Two genes (SCR1 and SCR2) encoding natural cycloheximide resistance in  the budding yeast Schwanniomyces occidentalis have been cloned by expression  in Saccharomyces cerevisiae.	gene_phenotype
71147	1	334221	7	NULL	NULL	0	NULL	SCR1	GP		is present in					Sw. occidentalis	Organism				NULL		0	NULL	NULL	NULL	gw70_yeast_19_9_735_s_34	12112229	Previously, we reported that two genes ( SCR1 and  SCR2) from the budding yeast  Sw. occidentalis were cloned and expressed in  S. cerevisiae (del Pozo  et al., [ 1993]).	gene_phenotype
71148	2	334221	7	NULL	NULL	0	NULL	SCR2	GP		is present in					Sw. occidentalis	Organism				NULL		0	NULL	NULL	NULL	gw70_yeast_19_9_735_s_34	12112229	Previously, we reported that two genes ( SCR1 and  SCR2) from the budding yeast  Sw. occidentalis were cloned and expressed in  S. cerevisiae (del Pozo  et al., [ 1993]).	gene_phenotype
71149	3	334221	7	NULL	NULL	0	NULL	Sw. occidentalis	Organism		is a type of					budding yeast	Organism				NULL		0	NULL	NULL	NULL	gw70_yeast_19_9_735_s_34	12112229	Previously, we reported that two genes ( SCR1 and  SCR2) from the budding yeast  Sw. occidentalis were cloned and expressed in  S. cerevisiae (del Pozo  et al., [ 1993]).	gene_phenotype
71150	1	334222	7	NULL	NULL	0	NULL	competent SRP	GP		assemble with					nuclear export	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_48	11352936	Our results suggest that assembly of a nuclear export - competent SRP takes place in the nucleolus and requires the four "`core"' SRP proteins, which are actively imported into the nucleus by the ribosomal import pathway, as well as an intact scR1 3' end.	gene_phenotype
71151	2	334222	7	NULL	NULL	0	NULL	statement 1	Process		takes place in					nucleolus	CellComponent				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_48	11352936	Our results suggest that assembly of a nuclear export - competent SRP takes place in the nucleolus and requires the four "`core"' SRP proteins, which are actively imported into the nucleus by the ribosomal import pathway, as well as an intact scR1 3' end.	gene_phenotype
71152	3	334222	7	NULL	NULL	0	NULL	statement 1	Process		requires					four "`core"' SRP proteins	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_48	11352936	Our results suggest that assembly of a nuclear export - competent SRP takes place in the nucleolus and requires the four "`core"' SRP proteins, which are actively imported into the nucleus by the ribosomal import pathway, as well as an intact scR1 3' end.	gene_phenotype
71153	4	334222	7	NULL	NULL	0	NULL	four "`core"' SRP proteins	GP		imported into		actively			nucleus	CellComponent				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_48	11352936	Our results suggest that assembly of a nuclear export - competent SRP takes place in the nucleolus and requires the four "`core"' SRP proteins, which are actively imported into the nucleus by the ribosomal import pathway, as well as an intact scR1 3' end.	gene_phenotype
71154	5	334222	7	NULL	NULL	0	NULL	statement 4	Process		occur by					ribosomal import pathway	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_48	11352936	Our results suggest that assembly of a nuclear export - competent SRP takes place in the nucleolus and requires the four "`core"' SRP proteins, which are actively imported into the nucleus by the ribosomal import pathway, as well as an intact scR1 3' end.	gene_phenotype
71155	6	334222	7	NULL	NULL	0	NULL	statement 1	Process		requires					scR1	GP	intact	3' end		NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_48	11352936	Our results suggest that assembly of a nuclear export - competent SRP takes place in the nucleolus and requires the four "`core"' SRP proteins, which are actively imported into the nucleus by the ribosomal import pathway, as well as an intact scR1 3' end.	gene_phenotype
71156	1	334223	7	NULL	NULL	0	NULL	ts strain	Organism	mutated	cause					scR1	GP	inhibition of nuclear export of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_244	11352936	The mutated gene in this  ts strain which causes inhibiton of scR1 nuclear export was cloned by complementation and found to correspond to the essential nucleoporin Nsp1p ( Fig 8 A and data not shown).	gene_phenotype
71157	2	334223	7	NULL	NULL	0	NULL	Nsp1p	GP		is a type of					nucleoporin	CellComponent	essential			NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_244	11352936	The mutated gene in this  ts strain which causes inhibiton of scR1 nuclear export was cloned by complementation and found to correspond to the essential nucleoporin Nsp1p ( Fig 8 A and data not shown).	gene_phenotype
71158	3	334223	7	NULL	NULL	0	NULL	statement 1	Process		is because of					Nsp1p	GP	mutated			NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_244	11352936	The mutated gene in this  ts strain which causes inhibiton of scR1 nuclear export was cloned by complementation and found to correspond to the essential nucleoporin Nsp1p ( Fig 8 A and data not shown).	gene_phenotype
71159	1	334224	7	NULL	NULL	NULL	NULL	scR1	GP		does not accumulate at					permissive temperature					NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_283	11352936	No accumulation of scR1 was observed in these cells at the permissive, semi-, or nonpermissive temperatures, although polyadenylated RNA was found to accumulate under the latter two conditions ( Fig 9 B and data not shown).	gene_phenotype
71160	2	334224	7	NULL	NULL	0	NULL	scR1	GP		does not accumulate at					semi-permissive temperature					NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_283	11352936	No accumulation of scR1 was observed in these cells at the permissive, semi-, or nonpermissive temperatures, although polyadenylated RNA was found to accumulate under the latter two conditions ( Fig 9 B and data not shown).	gene_phenotype
71161	3	334224	7	NULL	NULL	0	NULL	scR1	GP		does not accumulate at					nonpermissive temperature					NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_283	11352936	No accumulation of scR1 was observed in these cells at the permissive, semi-, or nonpermissive temperatures, although polyadenylated RNA was found to accumulate under the latter two conditions ( Fig 9 B and data not shown).	gene_phenotype
71162	4	334224	7	NULL	NULL	0	NULL	polyadenylated RNA	NucleicAcid		accumulate at					semi-permissive temperature					NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_283	11352936	No accumulation of scR1 was observed in these cells at the permissive, semi-, or nonpermissive temperatures, although polyadenylated RNA was found to accumulate under the latter two conditions ( Fig 9 B and data not shown).	gene_phenotype
71163	5	334224	7	NULL	NULL	NULL	NULL	polyadenylated RNA	NucleicAcid		accumulate at					nonpermissive temperature					NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_283	11352936	No accumulation of scR1 was observed in these cells at the permissive, semi-, or nonpermissive temperatures, although polyadenylated RNA was found to accumulate under the latter two conditions ( Fig 9 B and data not shown).	gene_phenotype
71164	1	334225	7	NULL	NULL	0	NULL	Nsp1p	GP		is a subset of					nucleoporins	CellComponent				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_284	11352936	Taken together, these data provide evidence that a subset of nucleoporins, consisting of Nsp1p and Nup159p, is important for scR1 nuclear export, whereas other nucleoporins, such as Nup85p, seem to be less important.	gene_phenotype
71165	2	334225	7	NULL	NULL	NULL	NULL	Nup159p	GP		is a subset of					nucleoporins	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_284	11352936	Taken together, these data provide evidence that a subset of nucleoporins, consisting of Nsp1p and Nup159p, is important for scR1 nuclear export, whereas other nucleoporins, such as Nup85p, seem to be less important.	gene_phenotype
71166	3	334225	7	NULL	NULL	0	NULL	statement 1	Process		is required for					scR1	GP	nuclear export of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_284	11352936	Taken together, these data provide evidence that a subset of nucleoporins, consisting of Nsp1p and Nup159p, is important for scR1 nuclear export, whereas other nucleoporins, such as Nup85p, seem to be less important.	gene_phenotype
71167	4	334225	7	NULL	NULL	0	NULL	statement 2	Process		is required for					scR1	GP	nuclear export of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_284	11352936	Taken together, these data provide evidence that a subset of nucleoporins, consisting of Nsp1p and Nup159p, is important for scR1 nuclear export, whereas other nucleoporins, such as Nup85p, seem to be less important.	gene_phenotype
71168	5	334225	7	NULL	NULL	0	NULL	Nup85p	GP		is a subset of					nucleoporins	CellComponent				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_284	11352936	Taken together, these data provide evidence that a subset of nucleoporins, consisting of Nsp1p and Nup159p, is important for scR1 nuclear export, whereas other nucleoporins, such as Nup85p, seem to be less important.	gene_phenotype
71169	6	334225	7	NULL	NULL	0	NULL	Nup85p	GP		important for		less			scR1	GP	nuclear export of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_284	11352936	Taken together, these data provide evidence that a subset of nucleoporins, consisting of Nsp1p and Nup159p, is important for scR1 nuclear export, whereas other nucleoporins, such as Nup85p, seem to be less important.	gene_phenotype
71956	1	334227	11	NULL	NULL	0	NULL	 pre-SRP proteins	GP	absence of 	accumulate					scR1	GP	nuclear			NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_341	11352936	However, the fact that absence of any one of the pre-SRP proteins leads to nuclear accumulation of scR1 suggests that SRP export is more complex than simple NES export.	gene_phenotype
71957	2	334227	11	NULL	NULL	0	NULL	SRP export	Process		is complex than		possibly			NES export	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_341	11352936	However, the fact that absence of any one of the pre-SRP proteins leads to nuclear accumulation of scR1 suggests that SRP export is more complex than simple NES export.	gene_phenotype
71958	1	334228	11	NULL	NULL	0	NULL	CRM1	GP		mediate					U snRNA	NucleicAcid	nuclear export			NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_344	11352936	Alternatively, an adapter protein, similar to the recently identified PHAX, which is required for CRM1-mediated U snRNA nuclear export ( Ohno et al. 2000   ), might be necessary for scR1 nuclear export.	gene_phenotype
71959	2	334228	11	NULL	NULL	0	NULL	adapter protein	GP		required for					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_344	11352936	Alternatively, an adapter protein, similar to the recently identified PHAX, which is required for CRM1-mediated U snRNA nuclear export ( Ohno et al. 2000   ), might be necessary for scR1 nuclear export.	gene_phenotype
71960	3	334228	11	NULL	NULL	0	NULL	adapter protein	GP		necessary for		possibly			scR1 	GP	nuclear export			NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_344	11352936	Alternatively, an adapter protein, similar to the recently identified PHAX, which is required for CRM1-mediated U snRNA nuclear export ( Ohno et al. 2000   ), might be necessary for scR1 nuclear export.	gene_phenotype
71961	1	334229	11	NULL	NULL	0	NULL	scR1	GP	Newly transcribed	assemble with					Srp14p	GP				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_20_1256_s_183	11069106	Newly transcribed scR1 is assembled with Srp14p, Srp21p, Srp68p and Srp72p to form a core SRP that is a substrate for export to the cytoplasm through a route sensitive to inactivation of the NES-binding protein Xpo1p/Crm1p or lack of Yrb2p activity at low temperature.	gene_phenotype
71962	2	334229	11	NULL	NULL	0	NULL	statement 1	GP		assemble with					Srp21p	GP				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_20_1256_s_183	11069106	Newly transcribed scR1 is assembled with Srp14p, Srp21p, Srp68p and Srp72p to form a core SRP that is a substrate for export to the cytoplasm through a route sensitive to inactivation of the NES-binding protein Xpo1p/Crm1p or lack of Yrb2p activity at low temperature.	gene_phenotype
71963	3	334229	11	NULL	NULL	0	NULL	statement 2	GP		assemble with					Srp68p	GP				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_20_1256_s_183	11069106	Newly transcribed scR1 is assembled with Srp14p, Srp21p, Srp68p and Srp72p to form a core SRP that is a substrate for export to the cytoplasm through a route sensitive to inactivation of the NES-binding protein Xpo1p/Crm1p or lack of Yrb2p activity at low temperature.	gene_phenotype
71964	4	334229	11	NULL	NULL	0	NULL	statement 3	GP		assemble with					Srp72p	GP				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_20_1256_s_183	11069106	Newly transcribed scR1 is assembled with Srp14p, Srp21p, Srp68p and Srp72p to form a core SRP that is a substrate for export to the cytoplasm through a route sensitive to inactivation of the NES-binding protein Xpo1p/Crm1p or lack of Yrb2p activity at low temperature.	gene_phenotype
71965	5	334229	11	NULL	NULL	0	NULL	statement 4	GP		forms					core SRP	GP				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_20_1256_s_183	11069106	Newly transcribed scR1 is assembled with Srp14p, Srp21p, Srp68p and Srp72p to form a core SRP that is a substrate for export to the cytoplasm through a route sensitive to inactivation of the NES-binding protein Xpo1p/Crm1p or lack of Yrb2p activity at low temperature.	gene_phenotype
71966	6	334229	11	NULL	NULL	0	NULL	core SRP	GP		export to					cytoplasm	Cell Component				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_20_1256_s_183	11069106	Newly transcribed scR1 is assembled with Srp14p, Srp21p, Srp68p and Srp72p to form a core SRP that is a substrate for export to the cytoplasm through a route sensitive to inactivation of the NES-binding protein Xpo1p/Crm1p or lack of Yrb2p activity at low temperature.	gene_phenotype
71971	1	334233	11	NULL	NULL	0	NULL	Prp43p	GP	depletion	accumulate		transient			23S pre-rRNAs	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_21_9269_s_167	16227579	Prp43p depletion is accompanied by a transient accumulation of the 35S and 23S pre-rRNAs and a strong decrease in the steady-state levels of the 27SA2, 27SB, 20S, and 7S pre-rRNAs and of all mature rRNAs, while levels of Scr1 RNA or tRNA-trp were little affected (Fig.  1B and  1C).	gene_phenotype
71974	2	334233	11	NULL	NULL	0	NULL	Prp43p	GP	depletion	accumulate		transient			 35S	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_21_9269_s_167	16227579	Prp43p depletion is accompanied by a transient accumulation of the 35S and 23S pre-rRNAs and a strong decrease in the steady-state levels of the 27SA2, 27SB, 20S, and 7S pre-rRNAs and of all mature rRNAs, while levels of Scr1 RNA or tRNA-trp were little affected (Fig.  1B and  1C).	gene_phenotype
71976	3	334233	11	NULL	NULL	0	NULL	Prp43p	GP	depletion	decreases		strongly			27SA2	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_21_9269_s_167	16227579	Prp43p depletion is accompanied by a transient accumulation of the 35S and 23S pre-rRNAs and a strong decrease in the steady-state levels of the 27SA2, 27SB, 20S, and 7S pre-rRNAs and of all mature rRNAs, while levels of Scr1 RNA or tRNA-trp were little affected (Fig.  1B and  1C).	gene_phenotype
71977	4	334233	11	NULL	NULL	0	NULL	Prp43p	GP	depletion	decreases		strongly			 27SB	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_21_9269_s_167	16227579	Prp43p depletion is accompanied by a transient accumulation of the 35S and 23S pre-rRNAs and a strong decrease in the steady-state levels of the 27SA2, 27SB, 20S, and 7S pre-rRNAs and of all mature rRNAs, while levels of Scr1 RNA or tRNA-trp were little affected (Fig.  1B and  1C).	gene_phenotype
71978	5	334233	11	NULL	NULL	0	NULL	Prp43p	GP	depletion	decreases		strongly			20S	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_21_9269_s_167	16227579	Prp43p depletion is accompanied by a transient accumulation of the 35S and 23S pre-rRNAs and a strong decrease in the steady-state levels of the 27SA2, 27SB, 20S, and 7S pre-rRNAs and of all mature rRNAs, while levels of Scr1 RNA or tRNA-trp were little affected (Fig.  1B and  1C).	gene_phenotype
71980	6	334233	11	NULL	NULL	0	NULL	Prp43p	GP	depletion	decreases		strongly			7S pre-rRNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_21_9269_s_167	16227579	Prp43p depletion is accompanied by a transient accumulation of the 35S and 23S pre-rRNAs and a strong decrease in the steady-state levels of the 27SA2, 27SB, 20S, and 7S pre-rRNAs and of all mature rRNAs, while levels of Scr1 RNA or tRNA-trp were little affected (Fig.  1B and  1C).	gene_phenotype
71981	7	334233	11	NULL	NULL	0	NULL	Prp43p	GP	depletion	decreases		strongly			mature rRNAs	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_21_9269_s_167	16227579	Prp43p depletion is accompanied by a transient accumulation of the 35S and 23S pre-rRNAs and a strong decrease in the steady-state levels of the 27SA2, 27SB, 20S, and 7S pre-rRNAs and of all mature rRNAs, while levels of Scr1 RNA or tRNA-trp were little affected (Fig.  1B and  1C).	gene_phenotype
71982	8	334233	11	NULL	NULL	NULL	NULL	Prp43p	GP	depletion	not affected					Scr1 RNA	NucleicAcid	levels			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_21_9269_s_167	16227579	Prp43p depletion is accompanied by a transient accumulation of the 35S and 23S pre-rRNAs and a strong decrease in the steady-state levels of the 27SA2, 27SB, 20S, and 7S pre-rRNAs and of all mature rRNAs, while levels of Scr1 RNA or tRNA-trp were little affected (Fig.  1B and  1C).	gene_phenotype
71983	9	334233	11	NULL	NULL	0	NULL	Prp43p	GP	depletion	not affected					tRNA-trp	NucleicAcid	levels			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_21_9269_s_167	16227579	Prp43p depletion is accompanied by a transient accumulation of the 35S and 23S pre-rRNAs and a strong decrease in the steady-state levels of the 27SA2, 27SB, 20S, and 7S pre-rRNAs and of all mature rRNAs, while levels of Scr1 RNA or tRNA-trp were little affected (Fig.  1B and  1C).	gene_phenotype
72025	1	334235	11	NULL	NULL	NULL	NULL	soluble Crry	GP	mouse 	is					sCrry	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_115_9_2444_s_27	16127466	Because of the species-selective activity of complement-inhibitory proteins, we decided to construct a novel recombinant protein consisting of a mouse CR2-targeting moiety linked to mouse soluble Crry (sCrry), an inhibitor of C3 activation which is a structural and functional analog of human soluble CR1 (sCR1).	gene_phenotype
72026	2	334235	11	NULL	NULL	NULL	NULL	soluble Crry	GP	mouse 	is an inhibitor of					C3	GP				NULL		NULL	NULL	NULL	NULL	gw70_jclininvest_115_9_2444_s_27	16127466	Because of the species-selective activity of complement-inhibitory proteins, we decided to construct a novel recombinant protein consisting of a mouse CR2-targeting moiety linked to mouse soluble Crry (sCrry), an inhibitor of C3 activation which is a structural and functional analog of human soluble CR1 (sCR1).	gene_phenotype
72029	3	334235	11	NULL	NULL	0	NULL	soluble Crry	GP		 is an analog of		 structural;;functional 			soluble CR1	GP	human			NULL		0	NULL	NULL	NULL	gw70_jclininvest_115_9_2444_s_27	16127466	Because of the species-selective activity of complement-inhibitory proteins, we decided to construct a novel recombinant protein consisting of a mouse CR2-targeting moiety linked to mouse soluble Crry (sCrry), an inhibitor of C3 activation which is a structural and functional analog of human soluble CR1 (sCR1).	gene_phenotype
72031	4	334235	11	NULL	NULL	0	NULL	soluble CR1	GP		is					sCR1	GP				NULL		0	NULL	NULL	NULL	gw70_jclininvest_115_9_2444_s_27	16127466	Because of the species-selective activity of complement-inhibitory proteins, we decided to construct a novel recombinant protein consisting of a mouse CR2-targeting moiety linked to mouse soluble Crry (sCrry), an inhibitor of C3 activation which is a structural and functional analog of human soluble CR1 (sCR1).	gene_phenotype
72037	1	334237	11	NULL	NULL	0	NULL	Xpo1p	GP		Exports		 Nuclear			SRP-RNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_167	11352936	The Nuclear Export of the SRP-RNA Is Distinct from mRNA Export and Mediated by Xpo1p   o identify the nuclear export route of scR1, we localized SRP-RNA in strains with an impaired Ran cycle, i.e., the above mentioned  rna1-1 and  prp20-1 mutant cells ( Aebi et al. 1990   ;   Corbett et al. 1995   ).	gene_phenotype
72038	2	334237	11	NULL	NULL	0	NULL	SRP-RNA export	Process	Nuclear	 Is Distinct from					mRNA Export	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_167	11352936	The Nuclear Export of the SRP-RNA Is Distinct from mRNA Export and Mediated by Xpo1p   o identify the nuclear export route of scR1, we localized SRP-RNA in strains with an impaired Ran cycle, i.e., the above mentioned  rna1-1 and  prp20-1 mutant cells ( Aebi et al. 1990   ;   Corbett et al. 1995   ).	gene_phenotype
72044	1	334239	11	NULL	NULL	NULL	NULL	Nucleolar factors	GP		stimulates					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_309	11352936	Nucleolar factors, or even scR1 or the rRNA nascent transcripts themselves, respectively, may facilitate the release of cargo destined for this compartment, similar to the stimulated release of the yeast protein Npl3p from its nuclear import receptor Mtr10p through RNA binding ( Senger et al. 1998   ).	gene_phenotype
72045	2	334239	11	NULL	NULL	0	NULL	Mtr10p	GP		is a type of 					nuclear import receptor	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_309	11352936	Nucleolar factors, or even scR1 or the rRNA nascent transcripts themselves, respectively, may facilitate the release of cargo destined for this compartment, similar to the stimulated release of the yeast protein Npl3p from its nuclear import receptor Mtr10p through RNA binding ( Senger et al. 1998   ).	gene_phenotype
72046	3	334239	11	NULL	NULL	NULL	NULL	Npl3p protein	GP	yeast	released from					Mtr10p	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_309	11352936	Nucleolar factors, or even scR1 or the rRNA nascent transcripts themselves, respectively, may facilitate the release of cargo destined for this compartment, similar to the stimulated release of the yeast protein Npl3p from its nuclear import receptor Mtr10p through RNA binding ( Senger et al. 1998   ).	gene_phenotype
72047	4	334239	11	NULL	NULL	0	NULL	statement 3	Process		occurs through					RNA binding	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_309	11352936	Nucleolar factors, or even scR1 or the rRNA nascent transcripts themselves, respectively, may facilitate the release of cargo destined for this compartment, similar to the stimulated release of the yeast protein Npl3p from its nuclear import receptor Mtr10p through RNA binding ( Senger et al. 1998   ).	gene_phenotype
72048	5	334239	11	NULL	NULL	0	NULL	scR1	GP		stimulates					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_309	11352936	Nucleolar factors, or even scR1 or the rRNA nascent transcripts themselves, respectively, may facilitate the release of cargo destined for this compartment, similar to the stimulated release of the yeast protein Npl3p from its nuclear import receptor Mtr10p through RNA binding ( Senger et al. 1998   ).	gene_phenotype
72049	6	334239	11	NULL	NULL	0	NULL	rRNA	NucleicAcid	nascent transcripts	stimulates					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_309	11352936	Nucleolar factors, or even scR1 or the rRNA nascent transcripts themselves, respectively, may facilitate the release of cargo destined for this compartment, similar to the stimulated release of the yeast protein Npl3p from its nuclear import receptor Mtr10p through RNA binding ( Senger et al. 1998   ).	gene_phenotype
72050	7	334239	11	NULL	NULL	0	NULL	Nucleolar factors	GP		release		may			cargo	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_309	11352936	Nucleolar factors, or even scR1 or the rRNA nascent transcripts themselves, respectively, may facilitate the release of cargo destined for this compartment, similar to the stimulated release of the yeast protein Npl3p from its nuclear import receptor Mtr10p through RNA binding ( Senger et al. 1998   ).	gene_phenotype
72051	8	334239	11	NULL	NULL	0	NULL	scR1	GP		releases		may			cargo	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_309	11352936	Nucleolar factors, or even scR1 or the rRNA nascent transcripts themselves, respectively, may facilitate the release of cargo destined for this compartment, similar to the stimulated release of the yeast protein Npl3p from its nuclear import receptor Mtr10p through RNA binding ( Senger et al. 1998   ).	gene_phenotype
72053	9	334239	11	NULL	NULL	0	NULL	rRNA	NucleicAcid	nascent transcripts	release		may			cargo	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_153_4_745_s_309	11352936	Nucleolar factors, or even scR1 or the rRNA nascent transcripts themselves, respectively, may facilitate the release of cargo destined for this compartment, similar to the stimulated release of the yeast protein Npl3p from its nuclear import receptor Mtr10p through RNA binding ( Senger et al. 1998   ).	gene_phenotype
72091	1	334252	11	NULL	NULL	NULL	NULL	GLFs	GP	L. major;;C. neoformans	encoded					UGM	GP	 activity			NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_4_6_1147_s_142	15947206	UGM activity of  L. major and  C. neoformans GLFs.  To confirm directly that candidate  GLFs encoded UGM activity, we first expressed high levels of protein in  E. coli using the pET3a system.	gene_phenotype
72092	1	334253	11	NULL	NULL	0	NULL	mutS	GP	T. aquaticus	increases					spontaneous mutation	Process	frequency			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_9_5040_s_124	8617781	Whereas the pET3a vector alone yielded a mutation  frequency similar to that of the host  E. coli  BL21, the  presence of  T. aquaticus mutS  resulted in a 14.3-fold increase  in the frequency of spontaneous mutation.	gene_phenotype
72093	1	334266	11	NULL	NULL	0	NULL	thioredoxin	GP		is					trx	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_96_24_14061_s_123	10570198	rPfCHT1 was expressed as a thioredoxin (trx) fusion protein in the expression plasmid pET32b by using as host cells the  E. coli mutant nonreducing strain AD494, which allows for intracytoplasmic formation of disulfide bonds.	gene_phenotype
72094	2	334266	11	NULL	NULL	0	NULL	thioredoxin	GP		is a type of 					 fusion protein	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_96_24_14061_s_123	10570198	rPfCHT1 was expressed as a thioredoxin (trx) fusion protein in the expression plasmid pET32b by using as host cells the  E. coli mutant nonreducing strain AD494, which allows for intracytoplasmic formation of disulfide bonds.	gene_phenotype
72095	3	334266	11	NULL	NULL	0	NULL	rPfCHT1	GP		expressed as					thioredoxin	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_96_24_14061_s_123	10570198	rPfCHT1 was expressed as a thioredoxin (trx) fusion protein in the expression plasmid pET32b by using as host cells the  E. coli mutant nonreducing strain AD494, which allows for intracytoplasmic formation of disulfide bonds.	gene_phenotype
72096	1	334270	11	NULL	NULL	NULL	NULL	paraxanthine	Chemical		convert to					caffeine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_febslett_534_1_75_s_170	12527364	Although recombinant CtCS7 was produced in  E. coli soluble extract, only the thioredoxin (Trx) fusion protein from the pET32a system had weak activity to convert paraxanthine to caffeine in this assay system.	gene_phenotype
72097	2	334270	11	NULL	NULL	0	NULL	 thioredoxin	GP		has activity to 					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_534_1_75_s_170	12527364	Although recombinant CtCS7 was produced in  E. coli soluble extract, only the thioredoxin (Trx) fusion protein from the pET32a system had weak activity to convert paraxanthine to caffeine in this assay system.	gene_phenotype
72098	3	334270	11	NULL	NULL	0	NULL	 thioredoxin	GP		is					Trx	GP				NULL		0	NULL	NULL	NULL	gw60_febslett_534_1_75_s_170	12527364	Although recombinant CtCS7 was produced in  E. coli soluble extract, only the thioredoxin (Trx) fusion protein from the pET32a system had weak activity to convert paraxanthine to caffeine in this assay system.	gene_phenotype
72099	4	334270	11	NULL	NULL	0	NULL	thioredoxin	GP		is a type of 					fusion protein	GP				NULL		0	NULL	NULL	NULL	gw60_febslett_534_1_75_s_170	12527364	Although recombinant CtCS7 was produced in  E. coli soluble extract, only the thioredoxin (Trx) fusion protein from the pET32a system had weak activity to convert paraxanthine to caffeine in this assay system.	gene_phenotype
72100	1	334273	11	NULL	NULL	0	NULL	RepA protein	GP		binds to		specifically			oriV DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_15_5003_s_260	15262938	A protein preparation generated in the same way as for His-tagged RepA but with  E. coli BL21 cells containing an empty expression vector (pET30a) showed no binding activity (not shown), implying that the RepA protein specifically binds to  oriV DNA.	gene_phenotype
72101	1	334275	11	NULL	NULL	0	NULL	ApaH protein	GP	S. Typhimurium	had the					enzymic activity	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_35_32602_s_92	12824172	To confirm that the   S. Typhimurium ApaH and YgdP proteins had the enzymic activities  predicted from their sequences, they were cloned and expressed in  E.  coli BL21(DE3) cells: ApaH in pET15b as a His-tagged 33.6-kDa protein and  YgdP in pET32b as a His-tagged thioredoxin fusion protein of total mass 39.2  kDa.	gene_phenotype
72102	2	334275	11	NULL	NULL	NULL	NULL	YgdP protein	GP	S. Typhimurium	had the					enzymic activity	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_35_32602_s_92	12824172	To confirm that the   S. Typhimurium ApaH and YgdP proteins had the enzymic activities  predicted from their sequences, they were cloned and expressed in  E.  coli BL21(DE3) cells: ApaH in pET15b as a His-tagged 33.6-kDa protein and  YgdP in pET32b as a His-tagged thioredoxin fusion protein of total mass 39.2  kDa.	gene_phenotype
72103	1	334277	11	NULL	NULL	0	NULL	CRP1	GP	maize chloroplast	processing					petD RNA	NucleicAcid	chloroplast			NULL		0	NULL	NULL	NULL	gw60_pnas_99_16_10887_s_197	12136123	This hypothesis is supported by the involvement in RNA metabolism and/or translation of the very few PPR motif-containing proteins characterized so far: maize chloroplast CRP1, involved in chloroplast  petD RNA processing and  petD and  petA translation ( 37),  Chlamydomonas MCA1, required for the accumulation of the chloroplast  petA transcript ( 38), yeast PET309, required for the stability and translation of the  coxI mitochondrial mRNA ( 39), and  Drosophila BSF, which binds to and stabilizes the bicoid mRNA ( 40).	gene_phenotype
72104	2	334277	11	NULL	NULL	0	NULL	CRP1	GP	maize chloroplast	translate					petD	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_99_16_10887_s_197	12136123	This hypothesis is supported by the involvement in RNA metabolism and/or translation of the very few PPR motif-containing proteins characterized so far: maize chloroplast CRP1, involved in chloroplast  petD RNA processing and  petD and  petA translation ( 37),  Chlamydomonas MCA1, required for the accumulation of the chloroplast  petA transcript ( 38), yeast PET309, required for the stability and translation of the  coxI mitochondrial mRNA ( 39), and  Drosophila BSF, which binds to and stabilizes the bicoid mRNA ( 40).	gene_phenotype
72105	3	334277	11	NULL	NULL	0	NULL	CRP1	GP	maize chloroplast	translate					petA	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_99_16_10887_s_197	12136123	This hypothesis is supported by the involvement in RNA metabolism and/or translation of the very few PPR motif-containing proteins characterized so far: maize chloroplast CRP1, involved in chloroplast  petD RNA processing and  petD and  petA translation ( 37),  Chlamydomonas MCA1, required for the accumulation of the chloroplast  petA transcript ( 38), yeast PET309, required for the stability and translation of the  coxI mitochondrial mRNA ( 39), and  Drosophila BSF, which binds to and stabilizes the bicoid mRNA ( 40).	gene_phenotype
72106	4	334277	11	NULL	NULL	0	NULL	MCA1	GP	Chlamydomonas	accumulate					petA transcript	GP	chloroplast			NULL		0	NULL	NULL	NULL	gw60_pnas_99_16_10887_s_197	12136123	This hypothesis is supported by the involvement in RNA metabolism and/or translation of the very few PPR motif-containing proteins characterized so far: maize chloroplast CRP1, involved in chloroplast  petD RNA processing and  petD and  petA translation ( 37),  Chlamydomonas MCA1, required for the accumulation of the chloroplast  petA transcript ( 38), yeast PET309, required for the stability and translation of the  coxI mitochondrial mRNA ( 39), and  Drosophila BSF, which binds to and stabilizes the bicoid mRNA ( 40).	gene_phenotype
72107	5	334277	11	NULL	NULL	0	NULL	PET309	GP	yeast	stabilize 					coxI mRNA	NucleicAcid	mitochondrial 			NULL		0	NULL	NULL	NULL	gw60_pnas_99_16_10887_s_197	12136123	This hypothesis is supported by the involvement in RNA metabolism and/or translation of the very few PPR motif-containing proteins characterized so far: maize chloroplast CRP1, involved in chloroplast  petD RNA processing and  petD and  petA translation ( 37),  Chlamydomonas MCA1, required for the accumulation of the chloroplast  petA transcript ( 38), yeast PET309, required for the stability and translation of the  coxI mitochondrial mRNA ( 39), and  Drosophila BSF, which binds to and stabilizes the bicoid mRNA ( 40).	gene_phenotype
72108	6	334277	11	NULL	NULL	0	NULL	PET309	GP	yeast	translate					coxI mRNA	NucleicAcid	mitochondrial 			NULL		0	NULL	NULL	NULL	gw60_pnas_99_16_10887_s_197	12136123	This hypothesis is supported by the involvement in RNA metabolism and/or translation of the very few PPR motif-containing proteins characterized so far: maize chloroplast CRP1, involved in chloroplast  petD RNA processing and  petD and  petA translation ( 37),  Chlamydomonas MCA1, required for the accumulation of the chloroplast  petA transcript ( 38), yeast PET309, required for the stability and translation of the  coxI mitochondrial mRNA ( 39), and  Drosophila BSF, which binds to and stabilizes the bicoid mRNA ( 40).	gene_phenotype
72109	7	334277	11	NULL	NULL	0	NULL	BSF	GP	Drosophila 	binds to					bicoid mRNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_pnas_99_16_10887_s_197	12136123	This hypothesis is supported by the involvement in RNA metabolism and/or translation of the very few PPR motif-containing proteins characterized so far: maize chloroplast CRP1, involved in chloroplast  petD RNA processing and  petD and  petA translation ( 37),  Chlamydomonas MCA1, required for the accumulation of the chloroplast  petA transcript ( 38), yeast PET309, required for the stability and translation of the  coxI mitochondrial mRNA ( 39), and  Drosophila BSF, which binds to and stabilizes the bicoid mRNA ( 40).	gene_phenotype
72110	8	334277	11	NULL	NULL	0	NULL	BSF	GP	Drosophila	stabilizes					bicoid mRNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_pnas_99_16_10887_s_197	12136123	This hypothesis is supported by the involvement in RNA metabolism and/or translation of the very few PPR motif-containing proteins characterized so far: maize chloroplast CRP1, involved in chloroplast  petD RNA processing and  petD and  petA translation ( 37),  Chlamydomonas MCA1, required for the accumulation of the chloroplast  petA transcript ( 38), yeast PET309, required for the stability and translation of the  coxI mitochondrial mRNA ( 39), and  Drosophila BSF, which binds to and stabilizes the bicoid mRNA ( 40).	gene_phenotype
72111	1	334280	11	NULL	NULL	0	NULL	tlc1h strain	Cell		has					meiosis	Process	altered			NULL		0	NULL	NULL	NULL	gw60_embo_22_7_1688_s_138	12660174	The  tlc1h strain has altered meiosis.	gene_phenotype
72113	1	334289	11	NULL	NULL	0	NULL	TLC1	GP		is not required for		directly			telomeric silencing	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_355	9755194	Thus,  TLC1 is not directly required for telomeric silencing.	gene_phenotype
72114	1	334294	11	NULL	NULL	0	NULL	TLC1	GP		is not required for		normally 			telomeric silencing	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_538	9755194	Furthermore,  TLC1 interferes with the telomeric silencing factor when overexpressed, but  TLC1 is not normally required for its telomeric silencing function.	gene_phenotype
72115	1	334309	11	NULL	NULL	0	NULL	yku80	GP		suppresses					TLC1 overexpression	GP	on telomeric silencing			NULL		0	NULL	NULL	NULL	gw70_genesdev_17_19_2384_s_79	12975323	Isolation of a new  yku80 allele that suppresses the effect of  TLC1 overexpression on telomeric silencing.	gene_phenotype
72140	1	334311	11	NULL	NULL	0	NULL	slx8	GP	mutation	did not affect					telomere length	Chromosome	steady-state			NULL	TLC1+ cells	0	NULL	NULL	NULL	gw70_nucleicacidsres_34_2_506_s_167	16428246	slx8 mutation did not affect steady-state telomere length in  TLC1+ cells.	gene_phenotype
72141	1	334312	11	NULL	NULL	0	NULL	 yKu70/80	GP		interacts with 		possibly			TLC1	GP				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_7_2090_s_28	15824061	These observations suggest that the interaction of yKu70/80 with TLC1 is important for maintaining the telomere length.	gene_phenotype
72142	2	334312	11	NULL	NULL	0	NULL	statement 1	Process		maintain					telomere length	Chromosome				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_7_2090_s_28	15824061	These observations suggest that the interaction of yKu70/80 with TLC1 is important for maintaining the telomere length.	gene_phenotype
72143	1	334318	11	NULL	NULL	0	NULL	TLC1	GP		does not affect		directly			 telomeric silencing	Chromosome				NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_360	9755194	TLC1 does not appear to play a direct role in telomeric silencing.	gene_phenotype
72144	1	334319	11	NULL	NULL	0	NULL	EST2	GP		affect 					telomere length	Chromosome				NULL		0	NULL	NULL	NULL	gw60_cell_99_7_723_s_25	10619426	In this  organism, over 25 genes affect telomere length in addition to  EST2 and  TLC1.	gene_phenotype
72145	2	334319	11	NULL	NULL	0	NULL	TLC1	GP		affects					telomere length	Chromosome				NULL		0	NULL	NULL	NULL	gw60_cell_99_7_723_s_25	10619426	In this  organism, over 25 genes affect telomere length in addition to  EST2 and  TLC1.	gene_phenotype
72146	1	334326	11	NULL	NULL	0	NULL	TLC1	GP	overexpression of	 restores					telomere length	Chromosome	wild-type			NULL	 mtr10delta mutant	0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6046_s_91	12167699	(B) Overexpression of  TLC1 restored wild-type telomere length in the  mtr10delta mutant.	gene_phenotype
72166	1	334332	11	NULL	NULL	0	NULL	TLC1	GP	overexpression 	shortens					telomere length	Chromosome				NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_304	9755194	Only  TLC1 and  SIR4 overexpression had significant and reproducible effects of shortening telomere length, consistent with earlier reports for  TLC1 ( S INGER and GOTTSCHLING 1994   ).	gene_phenotype
72167	2	334332	11	NULL	NULL	0	NULL	SIR4	GP	overexpression of	shortens					telomere length	Chromosome				NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_304	9755194	Only  TLC1 and  SIR4 overexpression had significant and reproducible effects of shortening telomere length, consistent with earlier reports for  TLC1 ( S INGER and GOTTSCHLING 1994   ).	gene_phenotype
72168	1	334334	11	NULL	NULL	0	NULL	TLC1 RNA	NucleicAcid		accumulates					TLC1	GP	mature form			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_598_s_172	11160879	Both the integrity of the Sm site on the TLC1 RNA and the presence of at least two of the Sm proteins are needed for accumulation of the mature form of TLC1 ( 16).	gene_phenotype
72169	2	334334	11	NULL	NULL	0	NULL	Sm proteins	GP		accumulates					 TLC1	GP	mature form			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_598_s_172	11160879	Both the integrity of the Sm site on the TLC1 RNA and the presence of at least two of the Sm proteins are needed for accumulation of the mature form of TLC1 ( 16).	gene_phenotype
72170	1	334335	11	NULL	NULL	0	NULL	tel1	GP	mutation	has synergistic effect on					telomere-DSB fusions	Process				NULL	tel1 tlc1 cells	0	NULL	NULL	NULL	gw60_molcell_11_5_1379_s_92	12769860	The  tel1 and  tlc1 mutations had a synergistic effect on telomere-DSB fusions, which occurred in greater than 1 in 103 genomes in  tel1 tlc1 cells.	gene_phenotype
72171	2	334335	11	NULL	NULL	0	NULL	tlc1	GP	mutation	has synergistic effect on					telomere-DSB fusion	Process				NULL	tel1 tlc1 cells	0	NULL	NULL	NULL	gw60_molcell_11_5_1379_s_92	12769860	The  tel1 and  tlc1 mutations had a synergistic effect on telomere-DSB fusions, which occurred in greater than 1 in 103 genomes in  tel1 tlc1 cells.	gene_phenotype
72172	1	334344	11	NULL	NULL	0	NULL	RAD52	GP	loss of	does not affect					telomere length	Chromosome				NULL	S. cerevisiae	0	NULL	NULL	NULL	gw70_genesdev_18_15_1781_s_199	15289453	Thus, while loss of  RAD52 or  RAD51 does not affect telomere length in  S. cerevisiae, rad52 tlc1, rad51 tlc1, or rad52 est1 double mutant cells senesce at a faster rate than  tlc1 or  est1 single mutants (Lundblad and Blackburn 1993 ;	gene_phenotype
72173	2	334344	11	NULL	NULL	0	NULL	RAD51	GP	loss of	does not affect					telomere length	Chromosome				NULL	S. cerevisiae	0	NULL	NULL	NULL	gw70_genesdev_18_15_1781_s_199	15289453	Thus, while loss of  RAD52 or  RAD51 does not affect telomere length in  S. cerevisiae, rad52 tlc1, rad51 tlc1, or rad52 est1 double mutant cells senesce at a faster rate than  tlc1 or  est1 single mutants (Lundblad and Blackburn 1993 ;	gene_phenotype
72192	1	334351	11	NULL	NULL	0	NULL	Ku	GP		binds					TLC1 RNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_genesdev_17_19_2384_s_101	12975323	The mutation might reduce Ku's ability to bind TLC1 RNA, or the mutation might enhance Ku's interactions with other silencing factors, leaving its ability to bind TLC1 RNA unchanged.	gene_phenotype
72193	2	334351	11	NULL	NULL	0	NULL	Ku	GP	mutation	reduces					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_genesdev_17_19_2384_s_101	12975323	The mutation might reduce Ku's ability to bind TLC1 RNA, or the mutation might enhance Ku's interactions with other silencing factors, leaving its ability to bind TLC1 RNA unchanged.	gene_phenotype
72194	1	334352	11	NULL	NULL	0	NULL	Ku70/80	GP	budding yeast	interacts with					TLC1	GP			stem - loop region	NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_7_2090_s_26	15824061	It has been shown in budding yeast that Ku70/80 (yKu70/80) interacts with a stem - loop region of TLC1, and yeast harboring a  yKu80 allele that is defective for TLC1 binding possesses shortened telomeres ( ).	gene_phenotype
72195	1	334357	11	NULL	NULL	0	NULL	TLC1	GP		is a type of 					telomerase RNA gene	GP				NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_535	9755194	TLC1:   s described in our earlier work, overexpression of the telomerase RNA gene  TLC1 disrupts telomeric silencing specifically and causes shortening of the telomeric DNA tract ( S INGER and GOTTSCHLING 1994   ).	gene_phenotype
72196	2	334357	11	NULL	NULL	0	NULL	TLC1	GP	overexpression of	disrupts		specifically			telomeric silencing	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_535	9755194	TLC1:   s described in our earlier work, overexpression of the telomerase RNA gene  TLC1 disrupts telomeric silencing specifically and causes shortening of the telomeric DNA tract ( S INGER and GOTTSCHLING 1994   ).	gene_phenotype
72197	3	334357	11	NULL	NULL	0	NULL	TLC1	GP	overexpression of	shortens					telomeric DNA tract	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_535	9755194	TLC1:   s described in our earlier work, overexpression of the telomerase RNA gene  TLC1 disrupts telomeric silencing specifically and causes shortening of the telomeric DNA tract ( S INGER and GOTTSCHLING 1994   ).	gene_phenotype
72198	1	334358	11	NULL	NULL	0	NULL	TLC1	GP		 was not required for		directly 			silencing	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_536	9755194	In the present study, we found that  TLC1 was not directly required for silencing; strains without  TLC1 and with only half the normal length of telomeric DNA at the end of the chromosome were still silenced ( Table 3).	gene_phenotype
72199	1	334359	11	NULL	NULL	0	NULL	TLC1 RNA	NucleicAcid		interacting with					silencing factor	GP	telomere-specific			NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_537	9755194	From these results, we suggest that the loss of telomeric silencing when  TLC1 is overexpressed is not the consequence of telomere DNA shortening, but rather, that  TLC1 RNA is interacting with a telomere-specific silencing factor.	gene_phenotype
72200	2	334359	11	NULL	NULL	0	NULL	 TLC1	GP	overexpression of	leads to		possibly			telomeric silencing	Process	loss of			NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_537	9755194	From these results, we suggest that the loss of telomeric silencing when  TLC1 is overexpressed is not the consequence of telomere DNA shortening, but rather, that  TLC1 RNA is interacting with a telomere-specific silencing factor.	gene_phenotype
73131	3	334359	11	NULL	NULL	0	NULL	telomere DNA	NucleicAcid	shortening of	does not lead to					telomeric silencing	Process	loss of			NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_537	9755194	From these results, we suggest that the loss of telomeric silencing when  TLC1 is overexpressed is not the consequence of telomere DNA shortening, but rather, that  TLC1 RNA is interacting with a telomere-specific silencing factor.	gene_phenotype
73132	4	334359	11	NULL	NULL	0	NULL	statement 2	Process		is a consequence of					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_537	9755194	From these results, we suggest that the loss of telomeric silencing when  TLC1 is overexpressed is not the consequence of telomere DNA shortening, but rather, that  TLC1 RNA is interacting with a telomere-specific silencing factor.	gene_phenotype
72201	1	334361	11	NULL	NULL	0	NULL	TLC1 RNA	NucleicAcid		is a type of 					telomerase RNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_currbiol_8_3_177_s_86	9443919	In yeast, the telomerase RNA  TLC1 and the Est1, Est2, Est3, and Est4/Cdc13 proteins are each essential for maintenance of telomere length  in vivo   [17-19]  , but only Est2 and  TLC1 are essential for telomerase activity in cell lysates    [8,20,21]  .	gene_phenotype
72202	2	334361	11	NULL	NULL	0	NULL	TLC1 RNA	NucleicAcid		maintain					telomere length	Chromosome				NULL	In yeast;;in vivo	0	NULL	NULL	NULL	gw60_currbiol_8_3_177_s_86	9443919	In yeast, the telomerase RNA  TLC1 and the Est1, Est2, Est3, and Est4/Cdc13 proteins are each essential for maintenance of telomere length  in vivo   [17-19]  , but only Est2 and  TLC1 are essential for telomerase activity in cell lysates    [8,20,21]  .	gene_phenotype
72203	3	334361	11	NULL	NULL	0	NULL	Est1 protein	GP		maintain					telomere length	Chromosome				NULL	In yeast;;in vivo	0	NULL	NULL	NULL	gw60_currbiol_8_3_177_s_86	9443919	In yeast, the telomerase RNA  TLC1 and the Est1, Est2, Est3, and Est4/Cdc13 proteins are each essential for maintenance of telomere length  in vivo   [17-19]  , but only Est2 and  TLC1 are essential for telomerase activity in cell lysates    [8,20,21]  .	gene_phenotype
72204	4	334361	11	NULL	NULL	0	NULL	Est2 protein	GP		maintain					telomere length	Chromosome				NULL	In yeast;;in vivo	0	NULL	NULL	NULL	gw60_currbiol_8_3_177_s_86	9443919	In yeast, the telomerase RNA  TLC1 and the Est1, Est2, Est3, and Est4/Cdc13 proteins are each essential for maintenance of telomere length  in vivo   [17-19]  , but only Est2 and  TLC1 are essential for telomerase activity in cell lysates    [8,20,21]  .	gene_phenotype
72205	5	334361	11	NULL	NULL	0	NULL	Est3 protein	GP		maintain					telomere length	Chromosome				NULL	In yeast;;in vivo	0	NULL	NULL	NULL	gw60_currbiol_8_3_177_s_86	9443919	In yeast, the telomerase RNA  TLC1 and the Est1, Est2, Est3, and Est4/Cdc13 proteins are each essential for maintenance of telomere length  in vivo   [17-19]  , but only Est2 and  TLC1 are essential for telomerase activity in cell lysates    [8,20,21]  .	gene_phenotype
72206	6	334361	11	NULL	NULL	0	NULL	Est4/Cdc13 protein	GP		maintain					telomere length	Chromosome				NULL	In yeast;;in vivo	0	NULL	NULL	NULL	gw60_currbiol_8_3_177_s_86	9443919	In yeast, the telomerase RNA  TLC1 and the Est1, Est2, Est3, and Est4/Cdc13 proteins are each essential for maintenance of telomere length  in vivo   [17-19]  , but only Est2 and  TLC1 are essential for telomerase activity in cell lysates    [8,20,21]  .	gene_phenotype
72207	7	334361	11	NULL	NULL	0	NULL	Est2	GP		activates					 telomerase	GP				NULL	 in cell lysates	0	NULL	NULL	NULL	gw60_currbiol_8_3_177_s_86	9443919	In yeast, the telomerase RNA  TLC1 and the Est1, Est2, Est3, and Est4/Cdc13 proteins are each essential for maintenance of telomere length  in vivo   [17-19]  , but only Est2 and  TLC1 are essential for telomerase activity in cell lysates    [8,20,21]  .	gene_phenotype
72208	8	334361	11	NULL	NULL	0	NULL	TLC1 	GP		activates					telomerase	GP				NULL	 in cell lysates	0	NULL	NULL	NULL	gw60_currbiol_8_3_177_s_86	9443919	In yeast, the telomerase RNA  TLC1 and the Est1, Est2, Est3, and Est4/Cdc13 proteins are each essential for maintenance of telomere length  in vivo   [17-19]  , but only Est2 and  TLC1 are essential for telomerase activity in cell lysates    [8,20,21]  .	gene_phenotype
72209	1	334364	11	NULL	NULL	0	NULL	dnl4	GP	mutation	suppress		completely			telomere-DSB fusions	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_11_5_1379_s_142	12769860	Unlike the  dnl4 mutation,  exo1 did not completely suppress telomere-DSB fusions, whose frequency was significantly greater in  exo1 tlc1 and  exo1 tel1 tlc1 than in completely wild-type cells   (Figure 2E).	gene_phenotype
72210	2	334364	11	NULL	NULL	0	NULL	exo1	GP		did not suppress		completely 			telomere-DSB fusions	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_11_5_1379_s_142	12769860	Unlike the  dnl4 mutation,  exo1 did not completely suppress telomere-DSB fusions, whose frequency was significantly greater in  exo1 tlc1 and  exo1 tel1 tlc1 than in completely wild-type cells   (Figure 2E).	gene_phenotype
72211	1	334372	11	NULL	NULL	0	NULL	TLC1	GP		encodes					telomerase	NucleicAcid	RNA subunit			NULL		0	NULL	NULL	NULL	gw70_annurevgenet_34_0_331_s_1049	11092831	Interactions of TLC1 (which encodes  the RNA subunit of telomerase), TEL1, and MEC1 in regulating telomere length in the  yeast  Saccharomyces cerevisiae.	gene_phenotype
73133	2	334372	11	NULL	NULL	0	NULL	TLC1	GP	interaction of	regulates					telomere	Chromosome	length of			NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw70_annurevgenet_34_0_331_s_1049	11092831	Interactions of TLC1 (which encodes  the RNA subunit of telomerase), TEL1, and MEC1 in regulating telomere length in the  yeast  Saccharomyces cerevisiae.	gene_phenotype
73134	3	334372	11	NULL	NULL	0	NULL	TEL1	GP	interaction of	regulates					telomere	Chromosome	length of			NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw70_annurevgenet_34_0_331_s_1049	11092831	Interactions of TLC1 (which encodes  the RNA subunit of telomerase), TEL1, and MEC1 in regulating telomere length in the  yeast  Saccharomyces cerevisiae.	gene_phenotype
73135	4	334372	11	NULL	NULL	0	NULL	MEC1	GP	interaction of	regulates					telomere	Chromosome	length of			NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw70_annurevgenet_34_0_331_s_1049	11092831	Interactions of TLC1 (which encodes  the RNA subunit of telomerase), TEL1, and MEC1 in regulating telomere length in the  yeast  Saccharomyces cerevisiae.	gene_phenotype
72212	1	334374	11	NULL	NULL	0	NULL	EST2 gene	GP	S.cerevisiae	activates					telomerase	GP				NULL	in vivo	0	NULL	NULL	NULL	gw70_nucleicacidsres_34_2_407_s_15	16418502	In budding yeast  S.cerevisiae, at least five genes,  EST2,  TLC1,  EST1,  EST3 and  CDC13, are required for telomerase activity  in vivo.	gene_phenotype
72213	2	334374	11	NULL	NULL	0	NULL	TLC1 gene	GP	S.cerevisiae	activates					telomerase	GP				NULL	in vivo	0	NULL	NULL	NULL	gw70_nucleicacidsres_34_2_407_s_15	16418502	In budding yeast  S.cerevisiae, at least five genes,  EST2,  TLC1,  EST1,  EST3 and  CDC13, are required for telomerase activity  in vivo.	gene_phenotype
72214	3	334374	11	NULL	NULL	0	NULL	EST1 gene	GP	S. cerevisiae	activates					telomerase	GP				NULL	in vivo	0	NULL	NULL	NULL	gw70_nucleicacidsres_34_2_407_s_15	16418502	In budding yeast  S.cerevisiae, at least five genes,  EST2,  TLC1,  EST1,  EST3 and  CDC13, are required for telomerase activity  in vivo.	gene_phenotype
72215	4	334374	11	NULL	NULL	0	NULL	EST3 gene	GP	S. cerevisiae	activates					telomerase	GP				NULL	in vivo	0	NULL	NULL	NULL	gw70_nucleicacidsres_34_2_407_s_15	16418502	In budding yeast  S.cerevisiae, at least five genes,  EST2,  TLC1,  EST1,  EST3 and  CDC13, are required for telomerase activity  in vivo.	gene_phenotype
72216	5	334374	11	NULL	NULL	0	NULL	CDC13 gene	GP	S. cerevisiae	activates					telomerase	GP				NULL	in vivo	0	NULL	NULL	NULL	gw70_nucleicacidsres_34_2_407_s_15	16418502	In budding yeast  S.cerevisiae, at least five genes,  EST2,  TLC1,  EST1,  EST3 and  CDC13, are required for telomerase activity  in vivo.	gene_phenotype
72217	1	334381	11	NULL	NULL	0	NULL	Cdc13p	GP		is a type of 					telomeric component	Chromosome				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_4_1623_s_254	14742705	Hence, mutations of a telomeric component, Cdc13p, other than in the  TLC1 template also lead to a chromosome segregation defect.	gene_phenotype
72218	2	334381	11	NULL	NULL	NULL	NULL	Cdc13p	GP	mutations	leads to					chromosome segregation	Process	defective			NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_4_1623_s_254	14742705	Hence, mutations of a telomeric component, Cdc13p, other than in the  TLC1 template also lead to a chromosome segregation defect.	gene_phenotype
72219	1	334384	11	NULL	NULL	0	NULL	Ku	GP		regulates					telomere length	Chromosome				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_22_8202_s_270	14585978	Ku regulates telomere length, in part, via an interaction with a stem-loop structure present in TLC1, the telomerase RNA subunit ( ,  ).	gene_phenotype
72220	2	334384	11	NULL	NULL	0	NULL	Ku	GP		interacts with 					TLC1	GP			stem-loop	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_22_8202_s_270	14585978	Ku regulates telomere length, in part, via an interaction with a stem-loop structure present in TLC1, the telomerase RNA subunit ( ,  ).	gene_phenotype
72221	3	334384	11	NULL	NULL	0	NULL	statement 2	Process		leads to		partially			statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_22_8202_s_270	14585978	Ku regulates telomere length, in part, via an interaction with a stem-loop structure present in TLC1, the telomerase RNA subunit ( ,  ).	gene_phenotype
72222	1	334386	11	NULL	NULL	0	NULL	TLC1 RNA	NucleicAcid	Saccharomyces	binds to					Sm protein	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_6_3882_s_272	12458198	In contrast, the  Saccharomyces TLC1 RNA is bound by Sm proteins and requires the same proteins for accumulation ( ).	gene_phenotype
72223	2	334386	11	NULL	NULL	0	NULL	statement 1	Process		is required for 					accumulation	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_6_3882_s_272	12458198	In contrast, the  Saccharomyces TLC1 RNA is bound by Sm proteins and requires the same proteins for accumulation ( ).	gene_phenotype
72224	1	334387	11	NULL	NULL	0	NULL	Tlc1	GP	yeast	is a type of 					telomerase	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_102_32_11290_s_202	16040803	More relevant to our studies, Mtr10 was implicated in nuclear import of the RNA component of yeast telomerase, Tlc1 ( ).	gene_phenotype
72225	2	334387	11	NULL	NULL	0	NULL	Mtr10	GP		import		nuclear			Tlc1	GP	RNA component			NULL		0	NULL	NULL	NULL	gw70_pnas_102_32_11290_s_202	16040803	More relevant to our studies, Mtr10 was implicated in nuclear import of the RNA component of yeast telomerase, Tlc1 ( ).	gene_phenotype
72226	1	334388	11	NULL	NULL	0	NULL	 TLC1	GP		encodes					telomerase	GP	RNA subunit of			NULL		0	NULL	NULL	NULL	gw60_genesdev_15_14_1845_s_528	11459833	Interactions of  TLC1 (which encodes the RNA subunit of telomerase),  TEL1, and  MEC1 in regulating telomere length in the yeast  Saccharomyces cerevisiae.	gene_phenotype
72227	2	334388	11	NULL	NULL	NULL	NULL	TLC1	GP	Interactions of 	 regulate					telomere	Chromosome	length of			NULL	Saccharomyces cerevisiae	NULL	NULL	NULL	NULL	gw60_genesdev_15_14_1845_s_528	11459833	Interactions of  TLC1 (which encodes the RNA subunit of telomerase),  TEL1, and  MEC1 in regulating telomere length in the yeast  Saccharomyces cerevisiae.	gene_phenotype
72228	3	334388	11	NULL	NULL	NULL	NULL	TEL1	GP	interaction of	regulate					telomere	Chromosome	length of			NULL	Saccharomyces cerevisiae	NULL	NULL	NULL	NULL	gw60_genesdev_15_14_1845_s_528	11459833	Interactions of  TLC1 (which encodes the RNA subunit of telomerase),  TEL1, and  MEC1 in regulating telomere length in the yeast  Saccharomyces cerevisiae.	gene_phenotype
72229	4	334388	11	NULL	NULL	NULL	NULL	MEC1	GP	interaction of	regulate					telomere	Chromosome	length of			NULL	Saccharomyces cerevisiae	NULL	NULL	NULL	NULL	gw60_genesdev_15_14_1845_s_528	11459833	Interactions of  TLC1 (which encodes the RNA subunit of telomerase),  TEL1, and  MEC1 in regulating telomere length in the yeast  Saccharomyces cerevisiae.	gene_phenotype
72230	1	334389	11	NULL	NULL	0	NULL	TLC1 RNA	NucleicAcid		influence		possibly			telomere clustering	Process	at the nuclear periphery			NULL		0	NULL	NULL	NULL	gw60_genetics_160_1_49_s_373	11805044	The possibility that  TLC1 RNA might also influence telomere clustering and/or localization at the nuclear periphery remains to be investigated.	gene_phenotype
72231	2	334389	11	NULL	NULL	0	NULL	TLC1 RNA	NucleicAcid		influence					localization	Process	at the nuclear periphery			NULL		0	NULL	NULL	NULL	gw60_genetics_160_1_49_s_373	11805044	The possibility that  TLC1 RNA might also influence telomere clustering and/or localization at the nuclear periphery remains to be investigated.	gene_phenotype
72232	1	334393	11	10	NULL	NULL	NULL	SIR4	GP	overexpression of	disrupts					telomeric silencing	Process				NULL		NULL	NULL	NULL	NULL	gw60_genetics_150_2_613_s_239	9755194	Overexpression of clones containing  SIR4,  DOT1,  TLC1,  ASF1,  DNA2, and  DOT4 each had a strong effect of disrupting telomeric silencing.	gene_phenotype
72233	2	334393	11	NULL	NULL	NULL	NULL	DOT1	GP	overexpression of	disrupts					telomeric silencing	Process				NULL		NULL	NULL	NULL	NULL	gw60_genetics_150_2_613_s_239	9755194	Overexpression of clones containing  SIR4,  DOT1,  TLC1,  ASF1,  DNA2, and  DOT4 each had a strong effect of disrupting telomeric silencing.	gene_phenotype
72234	3	334393	11	NULL	NULL	0	NULL	TLC1	GP	overexpression of	disrupts					telomeric silencing	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_239	9755194	Overexpression of clones containing  SIR4,  DOT1,  TLC1,  ASF1,  DNA2, and  DOT4 each had a strong effect of disrupting telomeric silencing.	gene_phenotype
72235	4	334393	11	NULL	NULL	0	NULL	ASF1	GP	Overexpression of	disrupts					telomeric silencing	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_239	9755194	Overexpression of clones containing  SIR4,  DOT1,  TLC1,  ASF1,  DNA2, and  DOT4 each had a strong effect of disrupting telomeric silencing.	gene_phenotype
72236	5	334393	11	NULL	NULL	0	NULL	DNA2	GP	overexpression of	disrupts					telomeric silencing	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_239	9755194	Overexpression of clones containing  SIR4,  DOT1,  TLC1,  ASF1,  DNA2, and  DOT4 each had a strong effect of disrupting telomeric silencing.	gene_phenotype
72237	6	334393	11	NULL	NULL	0	NULL	DOT4	GP	overexpression of	disrupts					telomeric silencing	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_239	9755194	Overexpression of clones containing  SIR4,  DOT1,  TLC1,  ASF1,  DNA2, and  DOT4 each had a strong effect of disrupting telomeric silencing.	gene_phenotype
72238	1	334394	11	NULL	NULL	0	NULL	TLC1 gene	GP	overexpression of	regulate					telomere length	Chromosome				NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_306	9755194	Thus, overexpression of only three  DOT genes,  TLC1,  SIR4, and  DOT5, affected telomere length regulation and telomeric silencing.	gene_phenotype
72239	2	334394	11	NULL	NULL	0	NULL	TLC1 gene	GP	overexpression of	affects					telomeric silencing	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_306	9755194	Thus, overexpression of only three  DOT genes,  TLC1,  SIR4, and  DOT5, affected telomere length regulation and telomeric silencing.	gene_phenotype
72240	3	334394	11	NULL	NULL	0	NULL	SIR4 gene	GP	overexpression of	regulate					telomere length	Chromosome				NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_306	9755194	Thus, overexpression of only three  DOT genes,  TLC1,  SIR4, and  DOT5, affected telomere length regulation and telomeric silencing.	gene_phenotype
72241	4	334394	11	NULL	NULL	0	NULL	SIR4 gene	GP	overexpression of	affects					telomeric silencing	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_306	9755194	Thus, overexpression of only three  DOT genes,  TLC1,  SIR4, and  DOT5, affected telomere length regulation and telomeric silencing.	gene_phenotype
72242	5	334394	11	NULL	NULL	0	NULL	DOT5 gene	GP	overexpression of	regulate					telomere length	Chromosome				NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_306	9755194	Thus, overexpression of only three  DOT genes,  TLC1,  SIR4, and  DOT5, affected telomere length regulation and telomeric silencing.	gene_phenotype
72243	6	334394	11	NULL	NULL	0	NULL	DOT5 gene	GP	overexpression of	affects					telomeric silencing	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_306	9755194	Thus, overexpression of only three  DOT genes,  TLC1,  SIR4, and  DOT5, affected telomere length regulation and telomeric silencing.	gene_phenotype
72244	7	334394	11	NULL	NULL	0	NULL	TLC1	GP		is a type of 					DOT gene	GP				NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_306	9755194	Thus, overexpression of only three  DOT genes,  TLC1,  SIR4, and  DOT5, affected telomere length regulation and telomeric silencing.	gene_phenotype
72245	8	334394	11	NULL	NULL	0	NULL	SIR4	GP		is a type of 					DOT gene	GP				NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_306	9755194	Thus, overexpression of only three  DOT genes,  TLC1,  SIR4, and  DOT5, affected telomere length regulation and telomeric silencing.	gene_phenotype
72246	9	334394	11	NULL	NULL	0	NULL	DOT5	GP		is a type of 					DOT genes	GP				NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_306	9755194	Thus, overexpression of only three  DOT genes,  TLC1,  SIR4, and  DOT5, affected telomere length regulation and telomeric silencing.	gene_phenotype
72247	1	334395	11	NULL	NULL	NULL	NULL	TLC1 	GP		encodes					template RNA	NucleicAcid				NULL	Saccharomyces cerevisiae	NULL	NULL	NULL	NULL	gw60_genetics_162_3_1101_s_19	12454059	In the budding yeast  Saccharomyces cerevisiae, the template RNA and the catalytic subunit are encoded by  TLC1 and  EST2, respectively ( S INGER and GOTTSCHLING 1994   ;	gene_phenotype
72248	2	334395	11	NULL	NULL	0	NULL	EST2	GP		encodes					catalytic subunit	GP				NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw60_genetics_162_3_1101_s_19	12454059	In the budding yeast  Saccharomyces cerevisiae, the template RNA and the catalytic subunit are encoded by  TLC1 and  EST2, respectively ( S INGER and GOTTSCHLING 1994   ;	gene_phenotype
73136	1	334401	11	NULL	NULL	0	NULL	Smd1 protein	GP		co-immunoprecipitates with					TLC1 RNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_nature_401_6749_177_s_55	10490028	Figure 3  HA-tagged Smd1 protein co-immunoprecipitates  TLC1 RNA and  in vitro telomerase activity.	gene_phenotype
72249	1	334409	11	NULL	NULL	0	NULL	GGA	GP		co localize with					TGN46	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_6_2385_s_388	12808037	We find that GGAs and p56 show good  colocalization with the TGN marker TGN46, as well as with other proteins  associated with the Golgi stack ( Figure 4,  g - i; our unpublished observations).	gene_phenotype
72250	2	334409	11	NULL	NULL	0	NULL	p56 	GP		co localize with					TGN46	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_6_2385_s_388	12808037	We find that GGAs and p56 show good  colocalization with the TGN marker TGN46, as well as with other proteins  associated with the Golgi stack ( Figure 4,  g - i; our unpublished observations).	gene_phenotype
72251	3	334409	11	NULL	NULL	0	NULL	TGN46	GP		is a type of 					TGN marker	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_6_2385_s_388	12808037	We find that GGAs and p56 show good  colocalization with the TGN marker TGN46, as well as with other proteins  associated with the Golgi stack ( Figure 4,  g - i; our unpublished observations).	gene_phenotype
72252	1	334415	11	NULL	NULL	0	NULL	TLC1	GP		encodes					telomerase	GP	RNA component			NULL	yeast	0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6065_s_16	10454554	In yeast, the RNA component of telomerase is encoded by  TLC1 ( 33), and the protein component with reverse transcriptase activity is encoded by  EST2 ( 16).	gene_phenotype
72253	2	334415	11	NULL	NULL	0	NULL	EST2	GP		encodes					telomerase	GP	protein component			NULL	yeast	0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6065_s_16	10454554	In yeast, the RNA component of telomerase is encoded by  TLC1 ( 33), and the protein component with reverse transcriptase activity is encoded by  EST2 ( 16).	gene_phenotype
72254	1	334417	11	NULL	NULL	0	NULL	Est1 protein	GP		coimmunoprecipitates with					Tlc1	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_6_1947_s_4	10688642	We previously showed that Est1 protein coimmunoprecipitates with Tlc1 (the telomerase RNA) as well as with telomerase activity.	gene_phenotype
72255	1	334425	11	NULL	NULL	0	NULL	Mtr10p	GP		functions in					nucleocytoplasmic transport	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6046_s_282	12167699	Because Mtr10p functions in nucleocytoplasmic transport, we used RNA FISH to ask whether Tlc1 localization was abnormal in  mtr10 mutants.	gene_phenotype
72256	1	334427	11	NULL	NULL	0	NULL	TLC1 gene	GP		encodes					telomerase RNA subunit	NucleicAcid				NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw60_molcellbiol_22_7_2366_s_11	11884619	In the budding yeast  Saccharomyces cerevisiae, the telomerase RNA subunit is approximately 1.3 kb and is encoded by the  TLC1 gene ( 38).	gene_phenotype
72258	1	334440	11	NULL	NULL	0	NULL	C3TA2 telomere	Chromosome		did not impair					chromosome stability	Process				NULL		0	NULL	NULL	NULL	gw70_embo_22_7_1688_s_216	12660174	Although the C3TA2 telomere did not impair chromosome stability, meiosis was compromised in the  tlc1h strain, as demonstrated by a paucity of four spore tetrads ( Figure 4B).	gene_phenotype
72260	2	334440	11	NULL	NULL	0	NULL	C3TA2 telomere	Chromosome		compromised					meiosis	Process				NULL	tlc1h strain	0	NULL	NULL	NULL	gw70_embo_22_7_1688_s_216	12660174	Although the C3TA2 telomere did not impair chromosome stability, meiosis was compromised in the  tlc1h strain, as demonstrated by a paucity of four spore tetrads ( Figure 4B).	gene_phenotype
72262	1	334441	11	NULL	NULL	0	NULL	Rap1	GP		is required for					meiosis	Process	efficient			NULL	S.pombe	0	NULL	NULL	NULL	gw70_embo_22_7_1688_s_217	12660174	Because Rap1 is required for efficient meiosis in  S.pombe ( ;  ), it is tempting to speculate that the meiotic defect of the  tlc1h strain is due to the lack of Rap1p at the C3TA2 telomere.	gene_phenotype
75851	1	334443	11	NULL	NULL	0	NULL	 C3TA2 telomere	GP		did not impair					chromosome stability	Process				NULL		0	NULL	NULL	NULL	gw60_embo_22_7_1688_s_213	12660174	Although the C3TA2 telomere did not impair chromosome stability, meiosis was compromised in the  tlc1h strain, as demonstrated by a paucity of four spore tetrads (Figure  4B).	gene_phenotype
75852	2	334443	11	NULL	NULL	0	NULL	tlc1h strain	Organism		compromised					meiosis	Process				NULL		0	NULL	NULL	NULL	gw60_embo_22_7_1688_s_213	12660174	Although the C3TA2 telomere did not impair chromosome stability, meiosis was compromised in the  tlc1h strain, as demonstrated by a paucity of four spore tetrads (Figure  4B).	gene_phenotype
72289	1	334444	11	NULL	NULL	0	NULL	TLC1 RNA	NucleicAcid	high levels of 	negatively affect		may			 Ku	GP				NULL		0	NULL	NULL	NULL	gw70_genesdev_17_19_2384_s_77	12975323	We reasoned that if high levels of TLC1 RNA negatively affect Ku, then it might be possible to identify alleles of Ku that would suppress the effects of  TLC1 overexpression and give rise to colonies that maintain telomeric silencing (i.e., remain pink and Ura-).	gene_phenotype
72294	1	334446	11	NULL	NULL	NULL	NULL	TLC1	GP		is a synonym of					telomerase RNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8729_s_250	14612413	In  S. cerevisiae, a mutation in the template domain of telomerase RNA,  TLC1, termed  tlc1- C476G, which reduces Rap1p in vitro binding affinity to the telomeric repeats by 300-fold, results in an increase in telomere length in a manner similar to that observed in  K. lactis ter1- Acc ( ) (Fig.  5, compare lanes 2 and 3 to lane 1).	gene_phenotype
72297	2	334446	11	NULL	NULL	0	NULL	Rap1p	GP	in vitro	binds to					 telomeric repeats	Chromosome				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8729_s_250	14612413	In  S. cerevisiae, a mutation in the template domain of telomerase RNA,  TLC1, termed  tlc1- C476G, which reduces Rap1p in vitro binding affinity to the telomeric repeats by 300-fold, results in an increase in telomere length in a manner similar to that observed in  K. lactis ter1- Acc ( ) (Fig.  5, compare lanes 2 and 3 to lane 1).	gene_phenotype
73137	3	334446	11	NULL	NULL	NULL	NULL	TLC1	GP	mutation of	is termed as				template domain	tlc1- C476G	GP				NULL	S. cerevisiae	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8729_s_250	14612413	In  S. cerevisiae, a mutation in the template domain of telomerase RNA,  TLC1, termed  tlc1- C476G, which reduces Rap1p in vitro binding affinity to the telomeric repeats by 300-fold, results in an increase in telomere length in a manner similar to that observed in  K. lactis ter1- Acc ( ) (Fig.  5, compare lanes 2 and 3 to lane 1).	gene_phenotype
73138	4	334446	11	NULL	NULL	NULL	NULL	Rap1p	GP		bind					telomeric repeats	GP				NULL	S. cerevisiae;;in vitro	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8729_s_250	14612413	In  S. cerevisiae, a mutation in the template domain of telomerase RNA,  TLC1, termed  tlc1- C476G, which reduces Rap1p in vitro binding affinity to the telomeric repeats by 300-fold, results in an increase in telomere length in a manner similar to that observed in  K. lactis ter1- Acc ( ) (Fig.  5, compare lanes 2 and 3 to lane 1).	gene_phenotype
73139	5	334446	11	NULL	NULL	0	NULL	tlc1- C476G	GP		reduces					statement 3	GP	affinity of			NULL	S. cerevisiae	0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8729_s_250	14612413	In  S. cerevisiae, a mutation in the template domain of telomerase RNA,  TLC1, termed  tlc1- C476G, which reduces Rap1p in vitro binding affinity to the telomeric repeats by 300-fold, results in an increase in telomere length in a manner similar to that observed in  K. lactis ter1- Acc ( ) (Fig.  5, compare lanes 2 and 3 to lane 1).	gene_phenotype
73140	6	334446	11	NULL	NULL	0	NULL	statement 4	GP		increases					telomere	Chromosome	length of			NULL	S. cerevisiae	0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8729_s_250	14612413	In  S. cerevisiae, a mutation in the template domain of telomerase RNA,  TLC1, termed  tlc1- C476G, which reduces Rap1p in vitro binding affinity to the telomeric repeats by 300-fold, results in an increase in telomere length in a manner similar to that observed in  K. lactis ter1- Acc ( ) (Fig.  5, compare lanes 2 and 3 to lane 1).	gene_phenotype
72304	1	334453	11	NULL	NULL	0	NULL	TR subunit TLC1	GP	overexpression of 	increases					telomerase activity	Process				NULL	budding yeast;;in cell extracts	0	NULL	NULL	NULL	gw70_embo_25_3_565_s_56	16424902	In budding yeast, overexpression of the TR subunit TLC1 together with the TERT subunit  Est2p also results in higher telomerase activity levels in cell extracts (  et al).	gene_phenotype
72305	2	334453	11	NULL	NULL	0	NULL	TERT subunit Est2p	GP	overexpression of	increases					telomerase activity	Process				NULL	budding yeast;;in cell extracts	0	NULL	NULL	NULL	gw70_embo_25_3_565_s_56	16424902	In budding yeast, overexpression of the TR subunit TLC1 together with the TERT subunit  Est2p also results in higher telomerase activity levels in cell extracts (  et al).	gene_phenotype
72309	3	334453	11	NULL	NULL	0	NULL	statement 1	GP		acts together with					statement 1	GP				NULL		0	NULL	NULL	NULL	gw70_embo_25_3_565_s_56	16424902	In budding yeast, overexpression of the TR subunit TLC1 together with the TERT subunit  Est2p also results in higher telomerase activity levels in cell extracts (  et al).	gene_phenotype
72315	1	334461	11	NULL	NULL	0	NULL	 Ku	GP		is a type of 					DNA repair protein	GP				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_7_2090_s_4	15824061	The interaction between the DNA repair protein Ku and the RNA component of telomerase (TLC1) in  Saccharomyces cerevisiae has been shown to be important for maintaining telomere length.	gene_phenotype
72316	2	334461	11	NULL	NULL	0	NULL	TLC1	GP		is a type of 					RNA component of telomerase	GP				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_7_2090_s_4	15824061	The interaction between the DNA repair protein Ku and the RNA component of telomerase (TLC1) in  Saccharomyces cerevisiae has been shown to be important for maintaining telomere length.	gene_phenotype
72317	3	334461	11	NULL	NULL	0	NULL	Ku	GP		interacts with 					TLC1	GP				NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw70_nucleicacidsres_33_7_2090_s_4	15824061	The interaction between the DNA repair protein Ku and the RNA component of telomerase (TLC1) in  Saccharomyces cerevisiae has been shown to be important for maintaining telomere length.	gene_phenotype
72318	4	334461	11	NULL	NULL	0	NULL	statement 3	Process		maintains					telomere length	Chromosome				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_7_2090_s_4	15824061	The interaction between the DNA repair protein Ku and the RNA component of telomerase (TLC1) in  Saccharomyces cerevisiae has been shown to be important for maintaining telomere length.	gene_phenotype
72321	1	334471	11	NULL	NULL	0	NULL	EST2	GP	Deletion	 shortens					 telomeres	Chromosome				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_2_837_s_22	14701754	Deletion of either  EST2 or  TLC1 causes a progressive shortening of telomeres and eventual loss of culture viability ( ) that is analogous to the replicative senescence of cultured human fibroblasts.	gene_phenotype
72322	2	334471	11	NULL	NULL	0	NULL	TLC1	GP	Deletion	shortens					telomere	GP				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_2_837_s_22	14701754	Deletion of either  EST2 or  TLC1 causes a progressive shortening of telomeres and eventual loss of culture viability ( ) that is analogous to the replicative senescence of cultured human fibroblasts.	gene_phenotype
72323	3	334471	11	NULL	NULL	0	NULL	statement 1	Process		is an alternative to 					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_2_837_s_22	14701754	Deletion of either  EST2 or  TLC1 causes a progressive shortening of telomeres and eventual loss of culture viability ( ) that is analogous to the replicative senescence of cultured human fibroblasts.	gene_phenotype
72324	4	334471	11	NULL	NULL	0	NULL	statement 1	Process		leads to					loss of culture viability	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_2_837_s_22	14701754	Deletion of either  EST2 or  TLC1 causes a progressive shortening of telomeres and eventual loss of culture viability ( ) that is analogous to the replicative senescence of cultured human fibroblasts.	gene_phenotype
72325	5	334471	11	NULL	NULL	0	NULL	statement 2	Process		leads to					loss of culture viability	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_2_837_s_22	14701754	Deletion of either  EST2 or  TLC1 causes a progressive shortening of telomeres and eventual loss of culture viability ( ) that is analogous to the replicative senescence of cultured human fibroblasts.	gene_phenotype
72326	1	334472	11	NULL	NULL	0	NULL	Ku	GP		regulate					telomere length	Chromosome				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_22_8202_s_23	14585978	First, Ku is required for telomere length regulation ( ), an activity that is mediated through a 48-nucleotide stem-loop structure of TLC1, the RNA subunit of yeast telomerase ( ,  ).	gene_phenotype
72328	2	334472	11	NULL	NULL	0	NULL	statement 1	Process		mediated through					 TLC1	GP	 stem-loop structure			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_22_8202_s_23	14585978	First, Ku is required for telomere length regulation ( ), an activity that is mediated through a 48-nucleotide stem-loop structure of TLC1, the RNA subunit of yeast telomerase ( ,  ).	gene_phenotype
73121	1	334475	11	NULL	NULL	0	NULL	telomerase activity	Process	loss of	correlates with					TERT protein	GP	reduced amount of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_6_3882_s_39	12458198	In addition, for mutations in these motifs, the extent of telomerase activity loss correlates with the extent of reduction in the amount of TERT protein and TERT-associated TLC1 RNA.	gene_phenotype
73122	2	334475	11	NULL	NULL	NULL	NULL	telomerase activity	Process	loss of	correlates with					statement 3	Process	reduced amount of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_6_3882_s_39	12458198	In addition, for mutations in these motifs, the extent of telomerase activity loss correlates with the extent of reduction in the amount of TERT protein and TERT-associated TLC1 RNA.	gene_phenotype
73123	3	334475	11	NULL	NULL	0	NULL	TLC1 RNA	NucleicAcid		associates with					TERT	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_6_3882_s_39	12458198	In addition, for mutations in these motifs, the extent of telomerase activity loss correlates with the extent of reduction in the amount of TERT protein and TERT-associated TLC1 RNA.	gene_phenotype
72353	1	334480	11	NULL	NULL	NULL	NULL	TLC1 RNA	NucleicAcid	 overexpression 	 reduce					telomere	Chromosome	length of			NULL	 yeast cell	NULL	NULL	NULL	NULL	gw60_genetics_160_1_49_s_361	11805044	Third, overexpression of  TLC1 RNA has been shown to cause a modest  reduction in average telomere lengths in yeast cells ( S INGER and GOTTSCHLING 1994   ).	gene_phenotype
75853	1	334484	11	NULL	NULL	0	NULL	DOT1 gene	GP		 reduced					silencing	Process	when overexpressed			NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_7	9755194	With the exception of  TLC1, all these genes, particularly  DOT1 and  DOT4, also reduced silencing at other repressed loci ( HM loci and rDNA) when overexpressed.	gene_phenotype
75854	2	334484	11	NULL	NULL	0	NULL	DOT4 gene	GP		reduced					silencing	Process	when overexpressed			NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_7	9755194	With the exception of  TLC1, all these genes, particularly  DOT1 and  DOT4, also reduced silencing at other repressed loci ( HM loci and rDNA) when overexpressed.	gene_phenotype
75855	3	334484	11	NULL	NULL	0	NULL	TLC1 gene	GP		not reduced					silencing	Process	when overexpressed			NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_7	9755194	With the exception of  TLC1, all these genes, particularly  DOT1 and  DOT4, also reduced silencing at other repressed loci ( HM loci and rDNA) when overexpressed.	gene_phenotype
73124	1	334486	11	NULL	NULL	0	NULL	TLC1	GP		regulates					telomere	Chromosome	length of			NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw60_nucleicacidsres_29_11_2382_s_572	11376157	56       Ritchie,K., Mallory,J. and Petes,T.D. (1999) Interactions of  TLC1,  TEL1 and  MEC1 in regulating telomere length in the yeast  Saccharomyces cerevisiae.	gene_phenotype
73125	2	334486	11	NULL	NULL	0	NULL	TEL1	GP		regulates					telomere	Chromosome	length of			NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw60_nucleicacidsres_29_11_2382_s_572	11376157	56       Ritchie,K., Mallory,J. and Petes,T.D. (1999) Interactions of  TLC1,  TEL1 and  MEC1 in regulating telomere length in the yeast  Saccharomyces cerevisiae.	gene_phenotype
73126	3	334486	11	NULL	NULL	0	NULL	MEC1	GP		regulates					telomere	Chromosome	length of			NULL	 Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw60_nucleicacidsres_29_11_2382_s_572	11376157	56       Ritchie,K., Mallory,J. and Petes,T.D. (1999) Interactions of  TLC1,  TEL1 and  MEC1 in regulating telomere length in the yeast  Saccharomyces cerevisiae.	gene_phenotype
75856	1	334490	11	NULL	NULL	0	NULL	telomeres	Chromosome	a small fraction	undergoes		possibly			catastrophic shortening	Process				NULL	in tel1 tlc1 cells	0	NULL	NULL	NULL	gw60_molcell_11_5_1379_s_134	12769860	[In new window] This finding suggests that in  tel1 tlc1 cells, a small fraction of telomeres undergoes catastrophic shortening, causing loss of chromosome end protection and fusion to a DSB.	gene_phenotype
75857	2	334490	11	NULL	NULL	0	NULL	statement 1	Process		losses					end protection	Process	chromosome			NULL		0	NULL	NULL	NULL	gw60_molcell_11_5_1379_s_134	12769860	[In new window] This finding suggests that in  tel1 tlc1 cells, a small fraction of telomeres undergoes catastrophic shortening, causing loss of chromosome end protection and fusion to a DSB.	gene_phenotype
75858	3	334490	11	NULL	NULL	0	NULL	statement 1	Process		causes					DSB fusion	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_11_5_1379_s_134	12769860	[In new window] This finding suggests that in  tel1 tlc1 cells, a small fraction of telomeres undergoes catastrophic shortening, causing loss of chromosome end protection and fusion to a DSB.	gene_phenotype
75859	1	334493	11	NULL	NULL	0	NULL	Telomere length	Chromosome	tlc1 rad50 double mutant	shortened					progressively	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_5_1819_s_159	11238918	Telomere length in the  tlc1 rad50 double mutant shortened progressively, and in two of three independent experiments only type I survivors were found.	gene_phenotype
72354	1	334497	11	NULL	NULL	0	NULL	TLC1	GP	Overexpression of	restore					telomere length	Chromosome	wild-type			NULL	mtr10delta cells	0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6046_s_206	12167699	Overexpression of  TLC1 restored wild-type telomere length in  mtr10delta cells, whereas no significant changes were observed with the other genes assayed (Fig.  2B).	gene_phenotype
75860	1	334498	11	NULL	NULL	0	NULL	 Tlc1 tail	GP		occurs in the 					nucleus	CellComponent				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6046_s_362	12167699	(A) tail of Tlc1 occurs in the nucleus, which supports the hypothesis that in yeast the Sm proteins follow an RNA-independent nuclear import pathway ( 2).	gene_phenotype
75861	1	334502	11	NULL	NULL	0	NULL	 meiosis	Process		produces					four viable spores	Cell Component	from YMY2			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_50_33360_s_147	9837911	After meiosis, four viable spores were produced from YMY2, indicating that spores bearing a  TLC1 gene disruption are viable, as previously reported ( 25).	gene_phenotype
73127	1	334503	11	NULL	NULL	0	NULL	SLX5	GP		is in complex with					SLX8	GP				NULL		0	NULL	NULL	NULL	abs-batch0580-0599_nucleic-acids-res_34_2_16428246_s_7	16428246	However, mutations in SLX5 or  SLX8, which encode proteins that function together in a complex that is  required for viability in sgs1 mutants, do speed the senescence of tlc1  mutants.	gene_phenotype
73128	2	334503	11	NULL	NULL	0	NULL	stat1	GP		is required for					sgs1	GP	viability of;;mutant			NULL		0	NULL	NULL	NULL	abs-batch0580-0599_nucleic-acids-res_34_2_16428246_s_7	16428246	However, mutations in SLX5 or  SLX8, which encode proteins that function together in a complex that is  required for viability in sgs1 mutants, do speed the senescence of tlc1  mutants.	gene_phenotype
73129	3	334503	11	NULL	NULL	0	NULL	stat1	GP		speed					tlc1	GP	senescence of;;mutant			NULL		0	NULL	NULL	NULL	abs-batch0580-0599_nucleic-acids-res_34_2_16428246_s_7	16428246	However, mutations in SLX5 or  SLX8, which encode proteins that function together in a complex that is  required for viability in sgs1 mutants, do speed the senescence of tlc1  mutants.	gene_phenotype
72355	1	334505	11	NULL	NULL	NULL	NULL	TLC1	GP	wild-type	maintains					telomere	Chromosome	length of			NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_31_6_1646_s_162	12626706	While the presence of wild-type  TLC1 allowed normal telomere length maintenance (266  plus-or-minus  18 nt,  n = 20), cells that had received an empty vector lacked telomerase activity and consequently had significantly shorter telomeres (179  plus-or-minus  34 nt,  n = 20, shorter than wild-type  TLC1 P < 0.001,  t-test) 25 generations after a plasmid containing wild-type  TLC1 had been shuffled out.	gene_phenotype
72356	1	334509	11	NULL	NULL	0	NULL	Rap1	GP		is required for					meiosis	Process	efficient			NULL	S.pombe	0	NULL	NULL	NULL	gw60_embo_22_7_1688_s_214	12660174	Because Rap1 is required for efficient meiosis in  S.pombe ( Chikashige and Hiraoka, 2001;  Kanoh and Ishikawa, 2001), it is tempting to speculate that the meiotic defect of the  tlc1h strain is due to the lack of Rap1p at the C3TA2 telomere.	gene_phenotype
73130	2	334509	11	NULL	NULL	0	NULL	tlc1h strain	GP	meiotic defect of	is due to		potentially			Rap1p	GP	lack of			NULL	C3TA2 telomere	0	NULL	NULL	NULL	gw60_embo_22_7_1688_s_214	12660174	Because Rap1 is required for efficient meiosis in  S.pombe ( Chikashige and Hiraoka, 2001;  Kanoh and Ishikawa, 2001), it is tempting to speculate that the meiotic defect of the  tlc1h strain is due to the lack of Rap1p at the C3TA2 telomere.	gene_phenotype
72357	1	334514	11	NULL	NULL	0	NULL	Ku protein	GP	mutant	does not bind					 TLC1 RNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_genesdev_17_19_2384_s_103	12975323	Unlike the wild-type protein, the mutant Ku protein had no detectable TLC1 RNA-binding activity; no shifted species were seen, even in the presence of high levels of mutant Ku protein ( Fig. 3A).	gene_phenotype
72358	2	334514	11	NULL	NULL	0	NULL	Ku protein	GP	wild-type	binds					TLC1 RNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_genesdev_17_19_2384_s_103	12975323	Unlike the wild-type protein, the mutant Ku protein had no detectable TLC1 RNA-binding activity; no shifted species were seen, even in the presence of high levels of mutant Ku protein ( Fig. 3A).	gene_phenotype
72359	1	334515	11	NULL	NULL	0	NULL	Ku protein	GP		interacts with 					TLC1 RNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_genesdev_17_19_2384_s_247	12975323	In addition to the protein-RNA interaction between Ku and TLC1, there is also a protein-protein interaction between Cdc13p and Est1p that is essential for telomerase activity in vivo (Evans and Lundblad 1999 ; Pennock et al. 2001 ).	gene_phenotype
72360	2	334515	11	NULL	NULL	0	NULL	Cdc13p protein	GP		interacts with 					Est1p protein	GP				NULL		0	NULL	NULL	NULL	gw70_genesdev_17_19_2384_s_247	12975323	In addition to the protein-RNA interaction between Ku and TLC1, there is also a protein-protein interaction between Cdc13p and Est1p that is essential for telomerase activity in vivo (Evans and Lundblad 1999 ; Pennock et al. 2001 ).	gene_phenotype
72361	3	334515	11	NULL	NULL	0	NULL	statement 2	Process		is essential for					telomerase activity	Process				NULL	in vivo	0	NULL	NULL	NULL	gw70_genesdev_17_19_2384_s_247	12975323	In addition to the protein-RNA interaction between Ku and TLC1, there is also a protein-protein interaction between Cdc13p and Est1p that is essential for telomerase activity in vivo (Evans and Lundblad 1999 ; Pennock et al. 2001 ).	gene_phenotype
72362	1	334516	11	NULL	NULL	0	NULL	Ku	GP	S. cerevisiae	 interacting with		directly 			TLC1	GP				NULL		0	NULL	NULL	NULL	gw70_genesdev_18_15_1781_s_168	15289453	One mechanism by which Ku functions at the telomere has been revealed by work showing that  S. cerevisiae Ku regulates telomere length by interacting directly with TLC1 (Peterson et al. 2001 ; Stellwagen et al. 2003 ).	gene_phenotype
72363	2	334516	11	NULL	NULL	0	NULL	statement 1	Process		regulate					telomere length	Chromosome				NULL		0	NULL	NULL	NULL	gw70_genesdev_18_15_1781_s_168	15289453	One mechanism by which Ku functions at the telomere has been revealed by work showing that  S. cerevisiae Ku regulates telomere length by interacting directly with TLC1 (Peterson et al. 2001 ; Stellwagen et al. 2003 ).	gene_phenotype
72364	1	334523	11	NULL	NULL	0	NULL	Ku70/80	GP		interacts with 					hTR	GP				NULL	budding yeast	0	NULL	NULL	NULL	gw70_nucleicacidsres_33_7_2090_s_80	15824061	Interaction of Ku70/80 with hTR   In budding yeast, genetic studies show that yKu70/80 interacts with a 48 nt (nucleotides 288 - 335) stem - loop region of the RNA template (TLC1) of yeast telomerase ( ).	gene_phenotype
72365	2	334523	11	NULL	NULL	0	NULL	 yKu70/80	GP		interacts with					TLC1 RNA	NucleicAcid	 stem - loop region			NULL	 yeast 	0	NULL	NULL	NULL	gw70_nucleicacidsres_33_7_2090_s_80	15824061	Interaction of Ku70/80 with hTR   In budding yeast, genetic studies show that yKu70/80 interacts with a 48 nt (nucleotides 288 - 335) stem - loop region of the RNA template (TLC1) of yeast telomerase ( ).	gene_phenotype
71967	1	334527	5	NULL	NULL	0	NULL	TLC1 template sequence	NucleicAcid		directs		normally			telomeric TG1 - 3 repeats	NucleicAcid	synthesis of			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_4_1623_s_20	14742705	The  TLC1 template sequence normally directs the synthesis of telomeric TG1 - 3 repeats, which contain specific DNA binding sites for proteins involved in telomere length regulation and protection.	gene_phenotype
71968	2	334527	5	NULL	NULL	0	NULL	telomeric TG1 - 3 repeats	NucleicAcid		is involved in					telomere length	PhysicalPhenomenon	regulation of			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_4_1623_s_20	14742705	The  TLC1 template sequence normally directs the synthesis of telomeric TG1 - 3 repeats, which contain specific DNA binding sites for proteins involved in telomere length regulation and protection.	gene_phenotype
71969	3	334527	5	NULL	NULL	0	NULL	telomeric TG1 - 3 repeats	NucleicAcid		is involved in					telomere length	PhysicalPhenomenon	protection of			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_4_1623_s_20	14742705	The  TLC1 template sequence normally directs the synthesis of telomeric TG1 - 3 repeats, which contain specific DNA binding sites for proteins involved in telomere length regulation and protection.	gene_phenotype
71970	1	334530	5	NULL	NULL	NULL	NULL	TLC1	NucleicAcid	complete deletion of	causes					cell cycle arrest	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_15_4_1623_s_256	14742705	Complete deletion of  TLC1 causes cell cycle arrest, activates a checkpoint (Enomoto  et al., 2002 ; IJpma and Greider, 2003 ), and causes chromosomal fusions when telomeres become short (Hackett  et al., 2001 ).	gene_phenotype
71972	2	334530	5	NULL	NULL	0	NULL	TLC1	NucleicAcid	complete deletion of	activates					checkpoint	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_4_1623_s_256	14742705	Complete deletion of  TLC1 causes cell cycle arrest, activates a checkpoint (Enomoto  et al., 2002 ; IJpma and Greider, 2003 ), and causes chromosomal fusions when telomeres become short (Hackett  et al., 2001 ).	gene_phenotype
71973	3	334530	5	NULL	NULL	0	NULL	TLC1	NucleicAcid	complete deletion of	causes					chromosomal fusions	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_4_1623_s_256	14742705	Complete deletion of  TLC1 causes cell cycle arrest, activates a checkpoint (Enomoto  et al., 2002 ; IJpma and Greider, 2003 ), and causes chromosomal fusions when telomeres become short (Hackett  et al., 2001 ).	gene_phenotype
71975	4	334530	5	NULL	NULL	0	NULL	telomere	Chromosome	short	leads to					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_4_1623_s_256	14742705	Complete deletion of  TLC1 causes cell cycle arrest, activates a checkpoint (Enomoto  et al., 2002 ; IJpma and Greider, 2003 ), and causes chromosomal fusions when telomeres become short (Hackett  et al., 2001 ).	gene_phenotype
71979	1	334536	5	NULL	NULL	0	NULL	Est2	GP		associate with					tlc1-62 RNA	NucleicAcid	mutant			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_17_7720_s_252	15314178	The telomere length of the  tlc1-62 strain was indistinguishable from that of a  TLC1 strain (Fig.  8B), and Est2 association with the  tlc1-62 mutant RNA was reduced by less than twofold (Fig.  8C).	gene_phenotype
71984	1	334541	5	NULL	NULL	0	NULL	Ku	GP		plays a role in					telomere length	PhysicalPhenomenon	regulation of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_22_8202_s_375	14585978	In contrast, Ku's role in telomere length regulation is mediated through an interaction with a stem-loop structure of the TLC1 RNA subunit of telomerase ( ,  ) and may additionally require a function provided by the Est1 telomerase subunit ( ).	gene_phenotype
71985	2	334541	5	NULL	NULL	0	NULL	Ku	GP		interacts with					telomerase	GP	stem-loop structure of	TLC1 RNA subunit		NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_22_8202_s_375	14585978	In contrast, Ku's role in telomere length regulation is mediated through an interaction with a stem-loop structure of the TLC1 RNA subunit of telomerase ( ,  ) and may additionally require a function provided by the Est1 telomerase subunit ( ).	gene_phenotype
71986	3	334541	5	NULL	NULL	0	NULL	statement 2	Process		mediates					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_22_8202_s_375	14585978	In contrast, Ku's role in telomere length regulation is mediated through an interaction with a stem-loop structure of the TLC1 RNA subunit of telomerase ( ,  ) and may additionally require a function provided by the Est1 telomerase subunit ( ).	gene_phenotype
71987	4	334541	5	NULL	NULL	NULL	NULL	statement 1	Process		requires		additionally			telomerase 	GP	function of	Est1 subunit		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_22_8202_s_375	14585978	In contrast, Ku's role in telomere length regulation is mediated through an interaction with a stem-loop structure of the TLC1 RNA subunit of telomerase ( ,  ) and may additionally require a function provided by the Est1 telomerase subunit ( ).	gene_phenotype
71988	1	334542	5	NULL	NULL	0	NULL	Tlc1	GP		is not ubiquitous within					obligate intracellular organisms	Organism				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_17_6261_s_24	16923893	However, the Tlc1 family of transporters is not ubiquitous within obligate intracellular organisms; it is absent from the genomes of  Coxiella,  Anaplasma, and  Ehrlichia spp., which grow inside host-derived vesicles.	gene_phenotype
71989	2	334542	5	NULL	NULL	0	NULL	Tlc1	GP		is a family of					transporters	GP				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_17_6261_s_24	16923893	However, the Tlc1 family of transporters is not ubiquitous within obligate intracellular organisms; it is absent from the genomes of  Coxiella,  Anaplasma, and  Ehrlichia spp., which grow inside host-derived vesicles.	gene_phenotype
71990	3	334542	5	NULL	NULL	0	NULL	Tlc1	GP		is absent from					Coxiella	Organism	genome of			NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_17_6261_s_24	16923893	However, the Tlc1 family of transporters is not ubiquitous within obligate intracellular organisms; it is absent from the genomes of  Coxiella,  Anaplasma, and  Ehrlichia spp., which grow inside host-derived vesicles.	gene_phenotype
71991	4	334542	5	NULL	NULL	0	NULL	Tlc1	GP		is absent from					Anaplasma	Organism	genome of			NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_17_6261_s_24	16923893	However, the Tlc1 family of transporters is not ubiquitous within obligate intracellular organisms; it is absent from the genomes of  Coxiella,  Anaplasma, and  Ehrlichia spp., which grow inside host-derived vesicles.	gene_phenotype
71992	5	334542	5	NULL	NULL	0	NULL	Tlc1	GP		is absent from					Ehrlichia spp.	Organism	genome of			NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_17_6261_s_24	16923893	However, the Tlc1 family of transporters is not ubiquitous within obligate intracellular organisms; it is absent from the genomes of  Coxiella,  Anaplasma, and  Ehrlichia spp., which grow inside host-derived vesicles.	gene_phenotype
71993	6	334542	5	NULL	NULL	0	NULL	Ehrlichia spp.	Organism		grow inside					host-derived vesicles	CellComponent				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_17_6261_s_24	16923893	However, the Tlc1 family of transporters is not ubiquitous within obligate intracellular organisms; it is absent from the genomes of  Coxiella,  Anaplasma, and  Ehrlichia spp., which grow inside host-derived vesicles.	gene_phenotype
71994	7	334542	5	NULL	NULL	0	NULL	Anaplasma	Organism		grow inside					host-derived vesicles	CellComponent				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_17_6261_s_24	16923893	However, the Tlc1 family of transporters is not ubiquitous within obligate intracellular organisms; it is absent from the genomes of  Coxiella,  Anaplasma, and  Ehrlichia spp., which grow inside host-derived vesicles.	gene_phenotype
71995	8	334542	5	NULL	NULL	0	NULL	Coxiella	Organism		grow inside					host-derived vesicles	CellComponent				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_17_6261_s_24	16923893	However, the Tlc1 family of transporters is not ubiquitous within obligate intracellular organisms; it is absent from the genomes of  Coxiella,  Anaplasma, and  Ehrlichia spp., which grow inside host-derived vesicles.	gene_phenotype
71996	1	334543	5	NULL	NULL	NULL	NULL	telomerase RNAs	NucleicAcid	Kluyveromyces budding yeast;;sequence of	is different from					TLC1	NucleicAcid	Saccharomyces;;sequence of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_27_10024_s_81	15226497	Kluyveromyces budding yeast telomerase RNAs are significantly different in sequence from  Saccharomyces TLC1, making them useful for studying some conserved elements ( ,  ) but essentially useless for beginning to deduce overall RNA secondary structure.	gene_phenotype
71997	1	334544	5	NULL	NULL	0	NULL	TLC1	NucleicAcid		associate with					Est1p	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_41_14713_s_81	15371596	A conserved bulged-stem structure previously identified in seven budding yeast TERs is necessary for association of TLC1 with Est1p, a TER holoenzyme component, and various mutations within this bulged-stem structure cause senescence ( ).	gene_phenotype
71998	2	334544	5	NULL	NULL	0	NULL	bulged-stem structure	PhysicalPhenomenon	conserved	is present in					TERs	GP	budding yeast			NULL		0	NULL	NULL	NULL	gw70_pnas_101_41_14713_s_81	15371596	A conserved bulged-stem structure previously identified in seven budding yeast TERs is necessary for association of TLC1 with Est1p, a TER holoenzyme component, and various mutations within this bulged-stem structure cause senescence ( ).	gene_phenotype
71999	3	334544	5	NULL	NULL	0	NULL	statement 2	Process		is necessary for					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_101_41_14713_s_81	15371596	A conserved bulged-stem structure previously identified in seven budding yeast TERs is necessary for association of TLC1 with Est1p, a TER holoenzyme component, and various mutations within this bulged-stem structure cause senescence ( ).	gene_phenotype
72000	4	334544	5	NULL	NULL	0	NULL	Est1p	GP		is a component of					TER holoenzyme	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_41_14713_s_81	15371596	A conserved bulged-stem structure previously identified in seven budding yeast TERs is necessary for association of TLC1 with Est1p, a TER holoenzyme component, and various mutations within this bulged-stem structure cause senescence ( ).	gene_phenotype
72001	5	334544	5	NULL	NULL	0	NULL	bulged-stem structure	PhysicalPhenomenon	mutation in	causes					senescence	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_101_41_14713_s_81	15371596	A conserved bulged-stem structure previously identified in seven budding yeast TERs is necessary for association of TLC1 with Est1p, a TER holoenzyme component, and various mutations within this bulged-stem structure cause senescence ( ).	gene_phenotype
72002	1	334545	5	NULL	NULL	NULL	NULL	telomerase	GP		maintains					telomere	Chromosome	length of			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_21_6127_s_12	11689452	Maintenance of telomere length and structure usually requires telomerase, which is comprised of a reverse transcriptase (TERT in mammals, Est2 in the yeast  Saccharomyces cerevisiae) and an RNA template (TR in mammals,  TLC1 in  S.cerevisiae).	gene_phenotype
72003	2	334545	5	NULL	NULL	0	NULL	telomerase	GP		maintains					telomere	Chromosome	structure of			NULL		0	NULL	NULL	NULL	gw60_embo_20_21_6127_s_12	11689452	Maintenance of telomere length and structure usually requires telomerase, which is comprised of a reverse transcriptase (TERT in mammals, Est2 in the yeast  Saccharomyces cerevisiae) and an RNA template (TR in mammals,  TLC1 in  S.cerevisiae).	gene_phenotype
72004	3	334545	5	NULL	NULL	0	NULL	telomerase	GP		comprise of					reverse transcriptase	GP				NULL		0	NULL	NULL	NULL	gw60_embo_20_21_6127_s_12	11689452	Maintenance of telomere length and structure usually requires telomerase, which is comprised of a reverse transcriptase (TERT in mammals, Est2 in the yeast  Saccharomyces cerevisiae) and an RNA template (TR in mammals,  TLC1 in  S.cerevisiae).	gene_phenotype
72005	4	334545	5	NULL	NULL	0	NULL	telomerase	GP		comprise of					RNA template	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_embo_20_21_6127_s_12	11689452	Maintenance of telomere length and structure usually requires telomerase, which is comprised of a reverse transcriptase (TERT in mammals, Est2 in the yeast  Saccharomyces cerevisiae) and an RNA template (TR in mammals,  TLC1 in  S.cerevisiae).	gene_phenotype
72006	5	334545	5	NULL	NULL	0	NULL	statement 3	Process		occurs along with					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_embo_20_21_6127_s_12	11689452	Maintenance of telomere length and structure usually requires telomerase, which is comprised of a reverse transcriptase (TERT in mammals, Est2 in the yeast  Saccharomyces cerevisiae) and an RNA template (TR in mammals,  TLC1 in  S.cerevisiae).	gene_phenotype
72007	6	334545	5	NULL	NULL	0	NULL	TERT	GP	mammals	is a type of					reverse transcriptase	GP				NULL		0	NULL	NULL	NULL	gw60_embo_20_21_6127_s_12	11689452	Maintenance of telomere length and structure usually requires telomerase, which is comprised of a reverse transcriptase (TERT in mammals, Est2 in the yeast  Saccharomyces cerevisiae) and an RNA template (TR in mammals,  TLC1 in  S.cerevisiae).	gene_phenotype
72008	7	334545	5	NULL	NULL	0	NULL	Est2	GP	Saccharomyces cerevisiae	is a type of					reverse transcriptase	GP				NULL		0	NULL	NULL	NULL	gw60_embo_20_21_6127_s_12	11689452	Maintenance of telomere length and structure usually requires telomerase, which is comprised of a reverse transcriptase (TERT in mammals, Est2 in the yeast  Saccharomyces cerevisiae) and an RNA template (TR in mammals,  TLC1 in  S.cerevisiae).	gene_phenotype
72009	8	334545	5	NULL	NULL	0	NULL	TR	NucleicAcid	mammals	is a type of					RNA template	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_embo_20_21_6127_s_12	11689452	Maintenance of telomere length and structure usually requires telomerase, which is comprised of a reverse transcriptase (TERT in mammals, Est2 in the yeast  Saccharomyces cerevisiae) and an RNA template (TR in mammals,  TLC1 in  S.cerevisiae).	gene_phenotype
72010	9	334545	5	NULL	NULL	0	NULL	TLC1	NucleicAcid	S. cerevisiae	is a type of					RNA template	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_embo_20_21_6127_s_12	11689452	Maintenance of telomere length and structure usually requires telomerase, which is comprised of a reverse transcriptase (TERT in mammals, Est2 in the yeast  Saccharomyces cerevisiae) and an RNA template (TR in mammals,  TLC1 in  S.cerevisiae).	gene_phenotype
72011	1	334546	5	NULL	NULL	0	NULL	TLC1	NucleicAcid		encodes					telomerase	GP			RNA subunit	NULL		0	NULL	NULL	NULL	gw60_embo_20_21_6127_s_406	11689452	Ritchie,K.B., Mallory,J.C. and Petes,T.D. (1999) Interactions of  TLC1 (which encodes the RNA subunit of telomerase),  TEL1, and  MEC1 in regulating telomere length in the yeast  Saccharomyces cerevisiae.	gene_phenotype
72012	2	334546	5	NULL	NULL	0	NULL	TLC1	NucleicAcid	intractions of	regulates					telomere	Chromosome	length of			NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw60_embo_20_21_6127_s_406	11689452	Ritchie,K.B., Mallory,J.C. and Petes,T.D. (1999) Interactions of  TLC1 (which encodes the RNA subunit of telomerase),  TEL1, and  MEC1 in regulating telomere length in the yeast  Saccharomyces cerevisiae.	gene_phenotype
72013	3	334546	5	NULL	NULL	0	NULL	TEL1	GP	intractions of	regulates					telomere	Chromosome	length of			NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw60_embo_20_21_6127_s_406	11689452	Ritchie,K.B., Mallory,J.C. and Petes,T.D. (1999) Interactions of  TLC1 (which encodes the RNA subunit of telomerase),  TEL1, and  MEC1 in regulating telomere length in the yeast  Saccharomyces cerevisiae.	gene_phenotype
72014	4	334546	5	NULL	NULL	NULL	NULL	MEC1	GP	intractions of	regulates					telomere	Chromosome	length of			NULL	Saccharomyces cerevisiae	NULL	NULL	NULL	NULL	gw60_embo_20_21_6127_s_406	11689452	Ritchie,K.B., Mallory,J.C. and Petes,T.D. (1999) Interactions of  TLC1 (which encodes the RNA subunit of telomerase),  TEL1, and  MEC1 in regulating telomere length in the yeast  Saccharomyces cerevisiae.	gene_phenotype
72015	1	334551	5	NULL	NULL	0	NULL	genome	NucleicAcid		is instable in					tel1 mec1 cells	Cell				NULL		0	NULL	NULL	NULL	gw60_genetics_161_2_493_s_126	12072449	The  tlc1 mutation had only modest (threefold) effects, indicating that the elevated rates of genome instability in the  tel1 mec1 cells are not solely attributable to a deficiency in telomere length regulation.	gene_phenotype
72016	2	334551	5	NULL	NULL	0	NULL	statement 1	Process	elevated rates of 	is not attributable to		solely 			telomere	Chromosome	deficiency of;;regulation of;;length of			NULL		0	NULL	NULL	NULL	gw60_genetics_161_2_493_s_126	12072449	The  tlc1 mutation had only modest (threefold) effects, indicating that the elevated rates of genome instability in the  tel1 mec1 cells are not solely attributable to a deficiency in telomere length regulation.	gene_phenotype
72017	1	334553	5	NULL	NULL	0	NULL	tlc1	NucleicAcid		is a synonym of					telomerase RNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_genetics_161_4_1437_s_411	12196391	In  S. cerevisiae, it was observed that telomerase RNA ( tlc1) deletion hastened the loss of viability of  tel1delta mec1delta cells, suggesting that telomerase activity allows cells to partially counteract telomere loss ( C HAN et al. 2001   ).	gene_phenotype
72018	2	334553	5	NULL	NULL	0	NULL	tlc1	NucleicAcid	deletion of	hasten					tel1delta mec1delta cells	Cell	loss of;;viability of			NULL		0	NULL	NULL	NULL	gw60_genetics_161_4_1437_s_411	12196391	In  S. cerevisiae, it was observed that telomerase RNA ( tlc1) deletion hastened the loss of viability of  tel1delta mec1delta cells, suggesting that telomerase activity allows cells to partially counteract telomere loss ( C HAN et al. 2001   ).	gene_phenotype
72019	3	334553	5	NULL	NULL	0	NULL	cells	Cell		counteract		partially			telomere	Chromosome	loss of			NULL		0	NULL	NULL	NULL	gw60_genetics_161_4_1437_s_411	12196391	In  S. cerevisiae, it was observed that telomerase RNA ( tlc1) deletion hastened the loss of viability of  tel1delta mec1delta cells, suggesting that telomerase activity allows cells to partially counteract telomere loss ( C HAN et al. 2001   ).	gene_phenotype
72020	4	334553	5	NULL	NULL	0	NULL	telomerase activity	Process		allows					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_161_4_1437_s_411	12196391	In  S. cerevisiae, it was observed that telomerase RNA ( tlc1) deletion hastened the loss of viability of  tel1delta mec1delta cells, suggesting that telomerase activity allows cells to partially counteract telomere loss ( C HAN et al. 2001   ).	gene_phenotype
72021	1	334559	5	NULL	NULL	0	NULL	TLC1 RNA	NucleicAcid	overexpression of	increases					ionizing radiation	PhysicalPhenomenon	resistance to			NULL		0	NULL	NULL	NULL	gw60_genetics_160_1_49_s_339	11805044	Overexpression of  TLC1 RNA increased resistance to ionizing radiation (thought to be primarily dependent on recombinational repair processes) to a lesser extent than to MMS, which produces lesions that are repaired by several pathways ( X IAO et al. 1996   ).	gene_phenotype
72022	2	334559	5	NULL	NULL	0	NULL	TLC1 RNA	NucleicAcid	overexpression of	increases					MMS	Chemical	resistance to			NULL		0	NULL	NULL	NULL	gw60_genetics_160_1_49_s_339	11805044	Overexpression of  TLC1 RNA increased resistance to ionizing radiation (thought to be primarily dependent on recombinational repair processes) to a lesser extent than to MMS, which produces lesions that are repaired by several pathways ( X IAO et al. 1996   ).	gene_phenotype
72023	3	334559	5	NULL	NULL	0	NULL	statement 1	Process		lesser than					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_160_1_49_s_339	11805044	Overexpression of  TLC1 RNA increased resistance to ionizing radiation (thought to be primarily dependent on recombinational repair processes) to a lesser extent than to MMS, which produces lesions that are repaired by several pathways ( X IAO et al. 1996   ).	gene_phenotype
72024	1	334560	5	NULL	NULL	0	NULL	TLC1	NucleicAcid	overexpression of	reduce					telomere	Chromosome	silencing of			NULL		0	NULL	NULL	NULL	gw60_genetics_160_1_49_s_370	11805044	TLC1 was originally identified as one of several genes that reduced silencing at telomeres (but not at internal mating type loci) when overexpressed ( S INGER and GOTTSCHLING 1994   ;   S INGER  et al. 1998   ).	gene_phenotype
72027	1	334562	5	NULL	NULL	0	NULL	DNA	NucleicAcid	recombination of	plays a role in		possibly			telomere	Chromosome	maintenance of			NULL		0	NULL	NULL	NULL	gw60_genetics_152_1_143_s_49	10224249	To understand the role of DNA recombination in telomere maintenance more completely, we examined telomere length in a set of isogenic yeast mutants of the  RAD52 epistasis group in both the absence and presence of the telomerase RNA component  TLC1.	gene_phenotype
72028	1	334568	5	NULL	NULL	0	NULL	DOT1	NucleicAcid		plays a role in		potentially			telomere	Chromosome	silencing of			NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_320	9755194	To ascertain whether any of the other  DOT genes are important for telomeric silencing, the genomic copy of  DOT1,  DOT4,  DOT5,  DOT6,  TLC1, or  ASF1 was deleted and the effect on silencing was examined.	gene_phenotype
72030	2	334568	5	NULL	NULL	0	NULL	DOT4	NucleicAcid		plays a role in		potentially			telomere	Chromosome	silencing of			NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_320	9755194	To ascertain whether any of the other  DOT genes are important for telomeric silencing, the genomic copy of  DOT1,  DOT4,  DOT5,  DOT6,  TLC1, or  ASF1 was deleted and the effect on silencing was examined.	gene_phenotype
72032	3	334568	5	NULL	NULL	0	NULL	DOT5	NucleicAcid		plays a role in		potentially			telomere	Chromosome	silencing of			NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_320	9755194	To ascertain whether any of the other  DOT genes are important for telomeric silencing, the genomic copy of  DOT1,  DOT4,  DOT5,  DOT6,  TLC1, or  ASF1 was deleted and the effect on silencing was examined.	gene_phenotype
72033	4	334568	5	NULL	NULL	0	NULL	DOT6	NucleicAcid		plays a role in		potentially			telomere	Chromosome	silencing of			NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_320	9755194	To ascertain whether any of the other  DOT genes are important for telomeric silencing, the genomic copy of  DOT1,  DOT4,  DOT5,  DOT6,  TLC1, or  ASF1 was deleted and the effect on silencing was examined.	gene_phenotype
72034	5	334568	5	NULL	NULL	0	NULL	TLC1	NucleicAcid		plays a role in		potentially			telomere	Chromosome	silencing of			NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_320	9755194	To ascertain whether any of the other  DOT genes are important for telomeric silencing, the genomic copy of  DOT1,  DOT4,  DOT5,  DOT6,  TLC1, or  ASF1 was deleted and the effect on silencing was examined.	gene_phenotype
72035	6	334568	5	NULL	NULL	0	NULL	ASF1	NucleicAcid		plays a role in		potentially			telomere	Chromosome	silencing of			NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_320	9755194	To ascertain whether any of the other  DOT genes are important for telomeric silencing, the genomic copy of  DOT1,  DOT4,  DOT5,  DOT6,  TLC1, or  ASF1 was deleted and the effect on silencing was examined.	gene_phenotype
72036	1	334569	5	NULL	NULL	NULL	NULL	dot4	GP		plays a role in					rDNA	NucleicAcid	silencing of			NULL		NULL	NULL	NULL	NULL	gw60_genetics_150_2_613_s_386	9755194	While  dot4 cells had slightly less rDNA silencing than wild-type cells, as judged by sensitivity to 5-FOA, deletion of  DOT1,  DOT5,  DOT6, and  TLC1 had no effect.	gene_phenotype
72039	2	334569	5	NULL	NULL	0	NULL	DOT1	GP	deletion of	does not effect					rDNA	NucleicAcid	silencing of			NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_386	9755194	While  dot4 cells had slightly less rDNA silencing than wild-type cells, as judged by sensitivity to 5-FOA, deletion of  DOT1,  DOT5,  DOT6, and  TLC1 had no effect.	gene_phenotype
72040	3	334569	5	NULL	NULL	0	NULL	DOT5	GP	deletion of	does not effect					rDNA	NucleicAcid	silencing of			NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_386	9755194	While  dot4 cells had slightly less rDNA silencing than wild-type cells, as judged by sensitivity to 5-FOA, deletion of  DOT1,  DOT5,  DOT6, and  TLC1 had no effect.	gene_phenotype
72041	4	334569	5	NULL	NULL	0	NULL	DOT6	GP	deletion of	does not effect					rDNA	NucleicAcid	silencing of			NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_386	9755194	While  dot4 cells had slightly less rDNA silencing than wild-type cells, as judged by sensitivity to 5-FOA, deletion of  DOT1,  DOT5,  DOT6, and  TLC1 had no effect.	gene_phenotype
72042	5	334569	5	NULL	NULL	0	NULL	TLC1	NucleicAcid	deletion of	does not effect					rDNA	NucleicAcid	silencing of			NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_386	9755194	While  dot4 cells had slightly less rDNA silencing than wild-type cells, as judged by sensitivity to 5-FOA, deletion of  DOT1,  DOT5,  DOT6, and  TLC1 had no effect.	gene_phenotype
72043	1	334570	5	NULL	NULL	0	NULL	Est1 protein	GP		co-immunoprecipitate with		potentially			telomerase 	GP			TLC1 RNA subunit	NULL		0	NULL	NULL	NULL	gw60_genetics_162_3_1101_s_211	12454059	To test this, each mutant Est1 protein was examined for the ability to co-immunoprecipitate the TLC1 telomerase RNA subunit ( Fig 5A and data not shown); a subset was also tested for association with enzyme activity ( Fig 5B).	gene_phenotype
72052	1	334571	5	NULL	NULL	0	NULL	stem-loop structure	NucleicAcid		is present in					telomerase	GP			TLC1 component	NULL		0	NULL	NULL	NULL	gw60_genetics_162_3_1101_s_362	12454059	Recent work from the Gottschling laboratory has shown that a 48-nt stem-loop structure in the TLC1 component of telomerase influences telomere length through the same pathway as Ku ( P ETERSON  et al. 2001   ).	gene_phenotype
72054	2	334571	5	NULL	NULL	0	NULL	statement 1	Process		influences					telomere	Chromosome	length of			NULL		0	NULL	NULL	NULL	gw60_genetics_162_3_1101_s_362	12454059	Recent work from the Gottschling laboratory has shown that a 48-nt stem-loop structure in the TLC1 component of telomerase influences telomere length through the same pathway as Ku ( P ETERSON  et al. 2001   ).	gene_phenotype
72055	1	334574	5	NULL	NULL	0	NULL	Est protein	GP		interacts with					TLC1	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_13_809_s_30	10898986	[In new window] This interaction between the Est proteins and TLC1 reflected an association with an active telomerase complex, since enzyme activity was identified in each of the Est protein IPs (  Figure 1b).	gene_phenotype
72056	2	334574	5	NULL	NULL	0	NULL	statement 1	Process		associate with					telomerase complex	GP	active			NULL		0	NULL	NULL	NULL	gw60_currbiol_10_13_809_s_30	10898986	[In new window] This interaction between the Est proteins and TLC1 reflected an association with an active telomerase complex, since enzyme activity was identified in each of the Est protein IPs (  Figure 1b).	gene_phenotype
72057	3	334574	5	NULL	NULL	0	NULL	Est protein	GP		activates					enzyme	GP				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_13_809_s_30	10898986	[In new window] This interaction between the Est proteins and TLC1 reflected an association with an active telomerase complex, since enzyme activity was identified in each of the Est protein IPs (  Figure 1b).	gene_phenotype
73594	1	334575	5	NULL	NULL	0	NULL	est1	GP	mutant	inactivates		catalytically			telomerase	GP				NULL		0	NULL	NULL	NULL	gw60_nature_411_6841_1073_s_18	11429610	Mutations that inactivated the catalytic activity of telomerase ( est1, est2, est3, cdc13-2, tlc1) or inactivated proteins that affect telomeres ( tel1, sir1-4, yku70, yku80, rif1, rif2) 6,  7 had no significant effect on the GCR rate.	gene_phenotype
73595	2	334575	5	NULL	NULL	0	NULL	est2	GP	mutant	inactivates		catalytically			telomerase	GP				NULL		0	NULL	NULL	NULL	gw60_nature_411_6841_1073_s_18	11429610	Mutations that inactivated the catalytic activity of telomerase ( est1, est2, est3, cdc13-2, tlc1) or inactivated proteins that affect telomeres ( tel1, sir1-4, yku70, yku80, rif1, rif2) 6,  7 had no significant effect on the GCR rate.	gene_phenotype
73596	3	334575	5	NULL	NULL	0	NULL	est3	GP	mutant	inactivates		catalytically			telomerase	GP				NULL		0	NULL	NULL	NULL	gw60_nature_411_6841_1073_s_18	11429610	Mutations that inactivated the catalytic activity of telomerase ( est1, est2, est3, cdc13-2, tlc1) or inactivated proteins that affect telomeres ( tel1, sir1-4, yku70, yku80, rif1, rif2) 6,  7 had no significant effect on the GCR rate.	gene_phenotype
73597	4	334575	5	NULL	NULL	0	NULL	cdc13-2	GP	mutant	inactivates		catalytically			telomerase	GP				NULL		0	NULL	NULL	NULL	gw60_nature_411_6841_1073_s_18	11429610	Mutations that inactivated the catalytic activity of telomerase ( est1, est2, est3, cdc13-2, tlc1) or inactivated proteins that affect telomeres ( tel1, sir1-4, yku70, yku80, rif1, rif2) 6,  7 had no significant effect on the GCR rate.	gene_phenotype
73598	5	334575	5	NULL	NULL	0	NULL	tlc1	GP	mutant	inactivates		catalytically			telomerase	GP				NULL		0	NULL	NULL	NULL	gw60_nature_411_6841_1073_s_18	11429610	Mutations that inactivated the catalytic activity of telomerase ( est1, est2, est3, cdc13-2, tlc1) or inactivated proteins that affect telomeres ( tel1, sir1-4, yku70, yku80, rif1, rif2) 6,  7 had no significant effect on the GCR rate.	gene_phenotype
73599	6	334575	5	NULL	NULL	0	NULL	tel1	GP	inactive	affects					telomerase	GP				NULL		0	NULL	NULL	NULL	gw60_nature_411_6841_1073_s_18	11429610	Mutations that inactivated the catalytic activity of telomerase ( est1, est2, est3, cdc13-2, tlc1) or inactivated proteins that affect telomeres ( tel1, sir1-4, yku70, yku80, rif1, rif2) 6,  7 had no significant effect on the GCR rate.	gene_phenotype
73600	7	334575	5	NULL	NULL	0	NULL	sir1-4	GP	inactive	affects					telomerase	GP				NULL		0	NULL	NULL	NULL	gw60_nature_411_6841_1073_s_18	11429610	Mutations that inactivated the catalytic activity of telomerase ( est1, est2, est3, cdc13-2, tlc1) or inactivated proteins that affect telomeres ( tel1, sir1-4, yku70, yku80, rif1, rif2) 6,  7 had no significant effect on the GCR rate.	gene_phenotype
73601	8	334575	5	NULL	NULL	0	NULL	yku70	GP	inactive	affects					telomerase	GP				NULL		0	NULL	NULL	NULL	gw60_nature_411_6841_1073_s_18	11429610	Mutations that inactivated the catalytic activity of telomerase ( est1, est2, est3, cdc13-2, tlc1) or inactivated proteins that affect telomeres ( tel1, sir1-4, yku70, yku80, rif1, rif2) 6,  7 had no significant effect on the GCR rate.	gene_phenotype
73602	9	334575	5	NULL	NULL	0	NULL	yku80	GP	inactive	affects					telomerase	GP				NULL		0	NULL	NULL	NULL	gw60_nature_411_6841_1073_s_18	11429610	Mutations that inactivated the catalytic activity of telomerase ( est1, est2, est3, cdc13-2, tlc1) or inactivated proteins that affect telomeres ( tel1, sir1-4, yku70, yku80, rif1, rif2) 6,  7 had no significant effect on the GCR rate.	gene_phenotype
73603	10	334575	5	NULL	NULL	0	NULL	rif1	GP	inactive	affects					telomerase	GP				NULL		0	NULL	NULL	NULL	gw60_nature_411_6841_1073_s_18	11429610	Mutations that inactivated the catalytic activity of telomerase ( est1, est2, est3, cdc13-2, tlc1) or inactivated proteins that affect telomeres ( tel1, sir1-4, yku70, yku80, rif1, rif2) 6,  7 had no significant effect on the GCR rate.	gene_phenotype
73604	11	334575	5	NULL	NULL	0	NULL	rif2	GP	inactive	affects					telomerase	GP				NULL		0	NULL	NULL	NULL	gw60_nature_411_6841_1073_s_18	11429610	Mutations that inactivated the catalytic activity of telomerase ( est1, est2, est3, cdc13-2, tlc1) or inactivated proteins that affect telomeres ( tel1, sir1-4, yku70, yku80, rif1, rif2) 6,  7 had no significant effect on the GCR rate.	gene_phenotype
73605	12	334575	5	NULL	NULL	0	NULL	statement 1	Process		does not effect		significantly			GCR	PhysicalPhenomenon	rate of			NULL		0	NULL	NULL	NULL	gw60_nature_411_6841_1073_s_18	11429610	Mutations that inactivated the catalytic activity of telomerase ( est1, est2, est3, cdc13-2, tlc1) or inactivated proteins that affect telomeres ( tel1, sir1-4, yku70, yku80, rif1, rif2) 6,  7 had no significant effect on the GCR rate.	gene_phenotype
73606	13	334575	5	NULL	NULL	0	NULL	statement 2	Process		does not effect		significantly			GCR	PhysicalPhenomenon	rate of			NULL		0	NULL	NULL	NULL	gw60_nature_411_6841_1073_s_18	11429610	Mutations that inactivated the catalytic activity of telomerase ( est1, est2, est3, cdc13-2, tlc1) or inactivated proteins that affect telomeres ( tel1, sir1-4, yku70, yku80, rif1, rif2) 6,  7 had no significant effect on the GCR rate.	gene_phenotype
73607	14	334575	5	NULL	NULL	0	NULL	statement 3	Process		does not effect		significantly			GCR	PhysicalPhenomenon	rate of			NULL		0	NULL	NULL	NULL	gw60_nature_411_6841_1073_s_18	11429610	Mutations that inactivated the catalytic activity of telomerase ( est1, est2, est3, cdc13-2, tlc1) or inactivated proteins that affect telomeres ( tel1, sir1-4, yku70, yku80, rif1, rif2) 6,  7 had no significant effect on the GCR rate.	gene_phenotype
73608	15	334575	5	NULL	NULL	0	NULL	statement 4	Process		does not effect		significantly			GCR	PhysicalPhenomenon	rate of			NULL		0	NULL	NULL	NULL	gw60_nature_411_6841_1073_s_18	11429610	Mutations that inactivated the catalytic activity of telomerase ( est1, est2, est3, cdc13-2, tlc1) or inactivated proteins that affect telomeres ( tel1, sir1-4, yku70, yku80, rif1, rif2) 6,  7 had no significant effect on the GCR rate.	gene_phenotype
73609	16	334575	5	NULL	NULL	0	NULL	statement 5	Process		does not effect		significantly			GCR	PhysicalPhenomenon	rate of			NULL		0	NULL	NULL	NULL	gw60_nature_411_6841_1073_s_18	11429610	Mutations that inactivated the catalytic activity of telomerase ( est1, est2, est3, cdc13-2, tlc1) or inactivated proteins that affect telomeres ( tel1, sir1-4, yku70, yku80, rif1, rif2) 6,  7 had no significant effect on the GCR rate.	gene_phenotype
73610	17	334575	5	NULL	NULL	0	NULL	statement 6	Process		does not effect		significantly			GCR	PhysicalPhenomenon	rate of			NULL		0	NULL	NULL	NULL	gw60_nature_411_6841_1073_s_18	11429610	Mutations that inactivated the catalytic activity of telomerase ( est1, est2, est3, cdc13-2, tlc1) or inactivated proteins that affect telomeres ( tel1, sir1-4, yku70, yku80, rif1, rif2) 6,  7 had no significant effect on the GCR rate.	gene_phenotype
73611	18	334575	5	NULL	NULL	0	NULL	statement 7	Process		does not effect		significantly			GCR	PhysicalPhenomenon	rate of			NULL		0	NULL	NULL	NULL	gw60_nature_411_6841_1073_s_18	11429610	Mutations that inactivated the catalytic activity of telomerase ( est1, est2, est3, cdc13-2, tlc1) or inactivated proteins that affect telomeres ( tel1, sir1-4, yku70, yku80, rif1, rif2) 6,  7 had no significant effect on the GCR rate.	gene_phenotype
73612	19	334575	5	NULL	NULL	0	NULL	statement 8	Process		does not effect		significantly			GCR	PhysicalPhenomenon	rate of			NULL		0	NULL	NULL	NULL	gw60_nature_411_6841_1073_s_18	11429610	Mutations that inactivated the catalytic activity of telomerase ( est1, est2, est3, cdc13-2, tlc1) or inactivated proteins that affect telomeres ( tel1, sir1-4, yku70, yku80, rif1, rif2) 6,  7 had no significant effect on the GCR rate.	gene_phenotype
73613	20	334575	5	NULL	NULL	0	NULL	statement 9	Process		does not effect		significantly			GCR	PhysicalPhenomenon	rate of			NULL		0	NULL	NULL	NULL	gw60_nature_411_6841_1073_s_18	11429610	Mutations that inactivated the catalytic activity of telomerase ( est1, est2, est3, cdc13-2, tlc1) or inactivated proteins that affect telomeres ( tel1, sir1-4, yku70, yku80, rif1, rif2) 6,  7 had no significant effect on the GCR rate.	gene_phenotype
73614	21	334575	5	NULL	NULL	0	NULL	statement 10	Process		does not effect		significantly			GCR	PhysicalPhenomenon	rate of			NULL		0	NULL	NULL	NULL	gw60_nature_411_6841_1073_s_18	11429610	Mutations that inactivated the catalytic activity of telomerase ( est1, est2, est3, cdc13-2, tlc1) or inactivated proteins that affect telomeres ( tel1, sir1-4, yku70, yku80, rif1, rif2) 6,  7 had no significant effect on the GCR rate.	gene_phenotype
73615	22	334575	5	NULL	NULL	0	NULL	statement 11	Process		does not effect		significantly			GCR	PhysicalPhenomenon	rate of			NULL		0	NULL	NULL	NULL	gw60_nature_411_6841_1073_s_18	11429610	Mutations that inactivated the catalytic activity of telomerase ( est1, est2, est3, cdc13-2, tlc1) or inactivated proteins that affect telomeres ( tel1, sir1-4, yku70, yku80, rif1, rif2) 6,  7 had no significant effect on the GCR rate.	gene_phenotype
72058	1	334577	5	NULL	NULL	NULL	NULL	Tlc1	GP	Chlamydia	transports					nucleotide triphosphates	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_6_1397_s_270	10684935	All four  Chlamydia genomes also encode two proteins known to be dedicated to the transport of nucleotide triphosphates, Tlc1 and Tlc2, both homologs of Tlc, an ATP/ADP translocase from the obligate intracellular parasite  Rickettsia prowazakii ( 38).	gene_phenotype
72059	2	334577	5	NULL	NULL	NULL	NULL	Tlc2	GP	Chlamydia	transports					nucleotide triphosphates	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_6_1397_s_270	10684935	All four  Chlamydia genomes also encode two proteins known to be dedicated to the transport of nucleotide triphosphates, Tlc1 and Tlc2, both homologs of Tlc, an ATP/ADP translocase from the obligate intracellular parasite  Rickettsia prowazakii ( 38).	gene_phenotype
72060	3	334577	5	NULL	NULL	NULL	NULL	Tlc1	GP	Chlamydia	is homologous to					Tlc	GP	Rickettsia prowazakii 			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_6_1397_s_270	10684935	All four  Chlamydia genomes also encode two proteins known to be dedicated to the transport of nucleotide triphosphates, Tlc1 and Tlc2, both homologs of Tlc, an ATP/ADP translocase from the obligate intracellular parasite  Rickettsia prowazakii ( 38).	gene_phenotype
72061	4	334577	5	NULL	NULL	0	NULL	Tlc2	GP	Chlamydia	is homologous to					ATP/ADP translocase	GP	Rickettsia prowazakii			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_6_1397_s_270	10684935	All four  Chlamydia genomes also encode two proteins known to be dedicated to the transport of nucleotide triphosphates, Tlc1 and Tlc2, both homologs of Tlc, an ATP/ADP translocase from the obligate intracellular parasite  Rickettsia prowazakii ( 38).	gene_phenotype
72062	5	334577	5	NULL	NULL	0	NULL	Rickettsia prowazakii	Organism		is a type of					obligate intracellular parasite	Organism				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_6_1397_s_270	10684935	All four  Chlamydia genomes also encode two proteins known to be dedicated to the transport of nucleotide triphosphates, Tlc1 and Tlc2, both homologs of Tlc, an ATP/ADP translocase from the obligate intracellular parasite  Rickettsia prowazakii ( 38).	gene_phenotype
72063	1	334578	5	NULL	NULL	0	NULL	Tlc1 protein	GP	C.trachomatis serovar L2	is homologous to					ATP/ADP tranlocase	GP				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_6_1397_s_271	10684935	The Tlc1 protein of  C.trachomatis serovar L2 is an ATP/ADP tranlocase, whereas the Tlc2 protein, although sharing a high degree of sequence similarity, is a more general NTP transporter, apparently utilizing an H+ pump to energize the process ( 39).	gene_phenotype
72064	2	334578	5	NULL	NULL	0	NULL	Tlc2 protein	GP	C.trachomatis serovar L2	is homologous to					NTP transporter	GP				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_6_1397_s_271	10684935	The Tlc1 protein of  C.trachomatis serovar L2 is an ATP/ADP tranlocase, whereas the Tlc2 protein, although sharing a high degree of sequence similarity, is a more general NTP transporter, apparently utilizing an H+ pump to energize the process ( 39).	gene_phenotype
72065	1	334579	5	NULL	NULL	0	NULL	Cbf5p	GP		is a type of					H/ACA snoRNP protein	GP				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_598_s_8	11160879	We show that the presence of the H/ACA snoRNP proteins Cbf5p, Nhp2p and Nop10p, but not Gar1p, is required for the accumulation of mature non-polyadenylated hTR in yeast, while accumulation of TLC1 RNA is not affected by the absence of any of these proteins.	gene_phenotype
72066	2	334579	5	NULL	NULL	0	NULL	Nhp2p 	GP		is a type of					H/ACA snoRNP protein	GP				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_598_s_8	11160879	We show that the presence of the H/ACA snoRNP proteins Cbf5p, Nhp2p and Nop10p, but not Gar1p, is required for the accumulation of mature non-polyadenylated hTR in yeast, while accumulation of TLC1 RNA is not affected by the absence of any of these proteins.	gene_phenotype
72067	3	334579	5	NULL	NULL	0	NULL	Nop10p	GP		is a type of					H/ACA snoRNP protein	GP				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_598_s_8	11160879	We show that the presence of the H/ACA snoRNP proteins Cbf5p, Nhp2p and Nop10p, but not Gar1p, is required for the accumulation of mature non-polyadenylated hTR in yeast, while accumulation of TLC1 RNA is not affected by the absence of any of these proteins.	gene_phenotype
72068	4	334579	5	NULL	NULL	0	NULL	Gar1p	GP		is a type of					H/ACA snoRNP protein	GP				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_598_s_8	11160879	We show that the presence of the H/ACA snoRNP proteins Cbf5p, Nhp2p and Nop10p, but not Gar1p, is required for the accumulation of mature non-polyadenylated hTR in yeast, while accumulation of TLC1 RNA is not affected by the absence of any of these proteins.	gene_phenotype
72069	5	334579	5	NULL	NULL	0	NULL	Cbf5p	GP	presence of	is required for					hTR	GP	accumulation of;;mature;;non-polyadenylated			NULL	yeast	0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_598_s_8	11160879	We show that the presence of the H/ACA snoRNP proteins Cbf5p, Nhp2p and Nop10p, but not Gar1p, is required for the accumulation of mature non-polyadenylated hTR in yeast, while accumulation of TLC1 RNA is not affected by the absence of any of these proteins.	gene_phenotype
72070	6	334579	5	NULL	NULL	NULL	NULL	Nhp2p	GP	presence of	is required for					hTR	GP	accumulation of;;mature;;non-polyadenylated			NULL	yeast	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_598_s_8	11160879	We show that the presence of the H/ACA snoRNP proteins Cbf5p, Nhp2p and Nop10p, but not Gar1p, is required for the accumulation of mature non-polyadenylated hTR in yeast, while accumulation of TLC1 RNA is not affected by the absence of any of these proteins.	gene_phenotype
72071	7	334579	5	NULL	NULL	0	NULL	Nop10p	GP	presence of	is required for					hTR	GP	accumulation of;;mature;;non-polyadenylated			NULL	yeast	0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_598_s_8	11160879	We show that the presence of the H/ACA snoRNP proteins Cbf5p, Nhp2p and Nop10p, but not Gar1p, is required for the accumulation of mature non-polyadenylated hTR in yeast, while accumulation of TLC1 RNA is not affected by the absence of any of these proteins.	gene_phenotype
72072	8	334579	5	NULL	NULL	0	NULL	Gar1p	GP	presence of	is not required for					hTR	GP	accumulation of;;mature;;non-polyadenylated			NULL	yeast	0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_598_s_8	11160879	We show that the presence of the H/ACA snoRNP proteins Cbf5p, Nhp2p and Nop10p, but not Gar1p, is required for the accumulation of mature non-polyadenylated hTR in yeast, while accumulation of TLC1 RNA is not affected by the absence of any of these proteins.	gene_phenotype
72073	9	334579	5	NULL	NULL	0	NULL	TLC1 RNA	NucleicAcid	accumulation of	is not affected by					Cbf5p	GP	absence of			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_598_s_8	11160879	We show that the presence of the H/ACA snoRNP proteins Cbf5p, Nhp2p and Nop10p, but not Gar1p, is required for the accumulation of mature non-polyadenylated hTR in yeast, while accumulation of TLC1 RNA is not affected by the absence of any of these proteins.	gene_phenotype
72074	10	334579	5	NULL	NULL	0	NULL	TLC1 RNA	NucleicAcid	accumulation of	is not affected by					Nhp2p	GP	absence of			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_598_s_8	11160879	We show that the presence of the H/ACA snoRNP proteins Cbf5p, Nhp2p and Nop10p, but not Gar1p, is required for the accumulation of mature non-polyadenylated hTR in yeast, while accumulation of TLC1 RNA is not affected by the absence of any of these proteins.	gene_phenotype
72075	11	334579	5	NULL	NULL	0	NULL	TLC1 RNA	NucleicAcid	accumulation of	is not affected by					Nop10p	GP	absence of			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_598_s_8	11160879	We show that the presence of the H/ACA snoRNP proteins Cbf5p, Nhp2p and Nop10p, but not Gar1p, is required for the accumulation of mature non-polyadenylated hTR in yeast, while accumulation of TLC1 RNA is not affected by the absence of any of these proteins.	gene_phenotype
72076	12	334579	5	NULL	NULL	0	NULL	TLC1 RNA	NucleicAcid	accumulation of	is not affected by					Gar1p	GP	absence of			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_598_s_8	11160879	We show that the presence of the H/ACA snoRNP proteins Cbf5p, Nhp2p and Nop10p, but not Gar1p, is required for the accumulation of mature non-polyadenylated hTR in yeast, while accumulation of TLC1 RNA is not affected by the absence of any of these proteins.	gene_phenotype
72077	1	334580	5	NULL	NULL	0	NULL	Sm protein	GP		bind					TLC1 RNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_598_s_173	11160879	Thus it seems that Sm protein binding to TLC1 RNA is required for its accumulation, just as assembly of H/ACA snoRNP proteins on the H/ACA domain of hTR is required for the accumulation of this RNA.	gene_phenotype
72078	2	334580	5	NULL	NULL	0	NULL	H/ACA snoRNP proteins	GP		assemble on					hTR	GP		H/ACA domain		NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_598_s_173	11160879	Thus it seems that Sm protein binding to TLC1 RNA is required for its accumulation, just as assembly of H/ACA snoRNP proteins on the H/ACA domain of hTR is required for the accumulation of this RNA.	gene_phenotype
72079	3	334580	5	NULL	NULL	0	NULL	statement 1	Process		is required for					TLC1 RNA	NucleicAcid	accumulation of			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_598_s_173	11160879	Thus it seems that Sm protein binding to TLC1 RNA is required for its accumulation, just as assembly of H/ACA snoRNP proteins on the H/ACA domain of hTR is required for the accumulation of this RNA.	gene_phenotype
72080	4	334580	5	NULL	NULL	0	NULL	statement 2	Process		is required for					TLC1 RNA	NucleicAcid	accumulation of			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_29_3_598_s_173	11160879	Thus it seems that Sm protein binding to TLC1 RNA is required for its accumulation, just as assembly of H/ACA snoRNP proteins on the H/ACA domain of hTR is required for the accumulation of this RNA.	gene_phenotype
72081	1	334587	5	NULL	NULL	0	NULL	TLC1	NucleicAcid		encodes					telomerase	GP			RNA subunit	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6065_s_4	10454554	Mutations of  TLC1 (encoding the RNA subunit of telomerase) result in strains that have continually shortening telomeres and a gradual loss of cell viability; survivors of senescence arise as a consequence of a Rad52p-dependent recombination events that amplify telomeric and subtelomeric repeats.	gene_phenotype
72082	2	334587	5	NULL	NULL	0	NULL	TLC1	NucleicAcid	mutant	results in					telomere	Chromosome	short			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6065_s_4	10454554	Mutations of  TLC1 (encoding the RNA subunit of telomerase) result in strains that have continually shortening telomeres and a gradual loss of cell viability; survivors of senescence arise as a consequence of a Rad52p-dependent recombination events that amplify telomeric and subtelomeric repeats.	gene_phenotype
72083	3	334587	5	NULL	NULL	0	NULL	TLC1	NucleicAcid	mutant	results in					cell viability	Process	gradual loss of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6065_s_4	10454554	Mutations of  TLC1 (encoding the RNA subunit of telomerase) result in strains that have continually shortening telomeres and a gradual loss of cell viability; survivors of senescence arise as a consequence of a Rad52p-dependent recombination events that amplify telomeric and subtelomeric repeats.	gene_phenotype
72084	4	334587	5	NULL	NULL	0	NULL	Rad52p-dependent recombination	Process		amplify					telomeric repeats	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6065_s_4	10454554	Mutations of  TLC1 (encoding the RNA subunit of telomerase) result in strains that have continually shortening telomeres and a gradual loss of cell viability; survivors of senescence arise as a consequence of a Rad52p-dependent recombination events that amplify telomeric and subtelomeric repeats.	gene_phenotype
72085	5	334587	5	NULL	NULL	0	NULL	Rad52p-dependent recombination	Process		amplify					ubtelomeric repeats	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6065_s_4	10454554	Mutations of  TLC1 (encoding the RNA subunit of telomerase) result in strains that have continually shortening telomeres and a gradual loss of cell viability; survivors of senescence arise as a consequence of a Rad52p-dependent recombination events that amplify telomeric and subtelomeric repeats.	gene_phenotype
72086	1	334588	5	NULL	NULL	0	NULL	MEC1	GP	mutation of	reduce					telomere	Chromosome	length of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6065_s_5	10454554	We show that a mutation in  MEC1 (a gene related in sequence to  TEL1 and  ATM) reduces telomere length and that  tel1 mec1 double mutant strains have a senescent phenotype similar to that found in  tlc1 strains.	gene_phenotype
72087	2	334588	5	NULL	NULL	0	NULL	MEC1 gene	GP		is related to					TEL1	GP	sequence of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6065_s_5	10454554	We show that a mutation in  MEC1 (a gene related in sequence to  TEL1 and  ATM) reduces telomere length and that  tel1 mec1 double mutant strains have a senescent phenotype similar to that found in  tlc1 strains.	gene_phenotype
72088	3	334588	5	NULL	NULL	0	NULL	MEC1 gene	GP		is related to					ATM	GP	sequence of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6065_s_5	10454554	We show that a mutation in  MEC1 (a gene related in sequence to  TEL1 and  ATM) reduces telomere length and that  tel1 mec1 double mutant strains have a senescent phenotype similar to that found in  tlc1 strains.	gene_phenotype
72089	4	334588	5	NULL	NULL	0	NULL	tel1 mec1 strain	Cell	double mutant	contains					senescent phenotype	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6065_s_5	10454554	We show that a mutation in  MEC1 (a gene related in sequence to  TEL1 and  ATM) reduces telomere length and that  tel1 mec1 double mutant strains have a senescent phenotype similar to that found in  tlc1 strains.	gene_phenotype
72090	5	334588	5	NULL	NULL	0	NULL	statement 4	Process		is similar to					tlc1 strains	Cell				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6065_s_5	10454554	We show that a mutation in  MEC1 (a gene related in sequence to  TEL1 and  ATM) reduces telomere length and that  tel1 mec1 double mutant strains have a senescent phenotype similar to that found in  tlc1 strains.	gene_phenotype
72174	1	334589	5	NULL	NULL	0	NULL	cell viability	Process		is associated with					telomeric repeats	NucleicAcid	loss of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6065_s_20	10454554	Although yeast strains with a mutation in  EST or  TLC1 genes undergo dramatic loss of cell viability associated with loss of telomeric repeats, fast-growing survivors arise within the mutant cultures ( 18,  19).	gene_phenotype
72175	3	334589	5	NULL	NULL	NULL	NULL	statement 2	Cell		undergoes					statement 1	Process	dramatic loss of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_6065_s_20	10454554	Although yeast strains with a mutation in  EST or  TLC1 genes undergo dramatic loss of cell viability associated with loss of telomeric repeats, fast-growing survivors arise within the mutant cultures ( 18,  19).	gene_phenotype
72176	2	334589	5	NULL	NULL	0	NULL	yeast strain	Cell		contains					EST gene	GP	mutant			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6065_s_20	10454554	Although yeast strains with a mutation in  EST or  TLC1 genes undergo dramatic loss of cell viability associated with loss of telomeric repeats, fast-growing survivors arise within the mutant cultures ( 18,  19).	gene_phenotype
72177	4	334589	5	NULL	NULL	0	NULL	yeast strain	Cell		contains					TLC1 gene	GP	mutant			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6065_s_20	10454554	Although yeast strains with a mutation in  EST or  TLC1 genes undergo dramatic loss of cell viability associated with loss of telomeric repeats, fast-growing survivors arise within the mutant cultures ( 18,  19).	gene_phenotype
72178	5	334589	5	NULL	NULL	0	NULL	statement 4	Cell		undergoes					statement 1	Process	dramatic loss of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6065_s_20	10454554	Although yeast strains with a mutation in  EST or  TLC1 genes undergo dramatic loss of cell viability associated with loss of telomeric repeats, fast-growing survivors arise within the mutant cultures ( 18,  19).	gene_phenotype
73584	1	334590	5	NULL	NULL	NULL	NULL	est1 gene	GP	mutation of;;yeast	shortens		continually			telomere	Chromosome				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_6065_s_108	10454554	[[            Mutations ]] in five yeast genes ( est1 to - 4 and  tlc1), including the RNA and protein subunits of telomerase, result in continually shortening telomeres and a senescent phenotype, a gradual loss of cell viability during vegetative subculturing ( 13,  19,  33).	gene_phenotype
73585	2	334590	5	NULL	NULL	0	NULL	est1 gene	GP	mutation of;;yeast	results in					senescent phenotype	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6065_s_108	10454554	[[            Mutations ]] in five yeast genes ( est1 to - 4 and  tlc1), including the RNA and protein subunits of telomerase, result in continually shortening telomeres and a senescent phenotype, a gradual loss of cell viability during vegetative subculturing ( 13,  19,  33).	gene_phenotype
73586	3	334590	5	NULL	NULL	0	NULL	est2 gene	GP	mutation of;;yeast	shortens		continually			telomere	Chromosome				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6065_s_108	10454554	[[            Mutations ]] in five yeast genes ( est1 to - 4 and  tlc1), including the RNA and protein subunits of telomerase, result in continually shortening telomeres and a senescent phenotype, a gradual loss of cell viability during vegetative subculturing ( 13,  19,  33).	gene_phenotype
73587	4	334590	5	NULL	NULL	0	NULL	est2 gene	GP	mutation of;;yeast	results in					senescent phenotype	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6065_s_108	10454554	[[            Mutations ]] in five yeast genes ( est1 to - 4 and  tlc1), including the RNA and protein subunits of telomerase, result in continually shortening telomeres and a senescent phenotype, a gradual loss of cell viability during vegetative subculturing ( 13,  19,  33).	gene_phenotype
73588	5	334590	5	NULL	NULL	0	NULL	est3 gene	GP	mutation of;;yeast	shortens		continually			telomere	Chromosome				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6065_s_108	10454554	[[            Mutations ]] in five yeast genes ( est1 to - 4 and  tlc1), including the RNA and protein subunits of telomerase, result in continually shortening telomeres and a senescent phenotype, a gradual loss of cell viability during vegetative subculturing ( 13,  19,  33).	gene_phenotype
73589	6	334590	5	NULL	NULL	0	NULL	est3 gene	GP	mutation of;;yeast	results in					senescent phenotype	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6065_s_108	10454554	[[            Mutations ]] in five yeast genes ( est1 to - 4 and  tlc1), including the RNA and protein subunits of telomerase, result in continually shortening telomeres and a senescent phenotype, a gradual loss of cell viability during vegetative subculturing ( 13,  19,  33).	gene_phenotype
73590	7	334590	5	NULL	NULL	0	NULL	est4 gene	GP	mutation of;;yeast	results in					senescent phenotype	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6065_s_108	10454554	[[            Mutations ]] in five yeast genes ( est1 to - 4 and  tlc1), including the RNA and protein subunits of telomerase, result in continually shortening telomeres and a senescent phenotype, a gradual loss of cell viability during vegetative subculturing ( 13,  19,  33).	gene_phenotype
73591	8	334590	5	NULL	NULL	0	NULL	senescent phenotype	PhysicalPhenomenon		loses		gradually			cell viability	Process				NULL	during vegetative subculturing	0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6065_s_108	10454554	[[            Mutations ]] in five yeast genes ( est1 to - 4 and  tlc1), including the RNA and protein subunits of telomerase, result in continually shortening telomeres and a senescent phenotype, a gradual loss of cell viability during vegetative subculturing ( 13,  19,  33).	gene_phenotype
73592	9	334590	5	NULL	NULL	0	NULL	tlc1 gene	GP	mutation of;;yeast	shortens		continually			telomere	Chromosome				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6065_s_108	10454554	[[            Mutations ]] in five yeast genes ( est1 to - 4 and  tlc1), including the RNA and protein subunits of telomerase, result in continually shortening telomeres and a senescent phenotype, a gradual loss of cell viability during vegetative subculturing ( 13,  19,  33).	gene_phenotype
73593	10	334590	5	NULL	NULL	0	NULL	tlc1 gene	GP	mutation of;;yeast	results in					senescent phenotype	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6065_s_108	10454554	[[            Mutations ]] in five yeast genes ( est1 to - 4 and  tlc1), including the RNA and protein subunits of telomerase, result in continually shortening telomeres and a senescent phenotype, a gradual loss of cell viability during vegetative subculturing ( 13,  19,  33).	gene_phenotype
72179	1	334592	5	NULL	NULL	NULL	NULL	EST1 gene	GP	mutation of	leads to					telomere	Chromosome	progressive shortening of			NULL	Saccharomyces cerevisiae	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_1947_s_19	10688642	For the yeast  Saccharomyces cerevisiae, genetic screens have identified five genes ( EST1,  EST2,  EST3,  EST4/CDC13, and  TLC1) ( 20,  27,  39) whose mutations lead to progressive telomere shortening and eventual loss of viability (i.e., senescence).	gene_phenotype
72180	2	334592	5	NULL	NULL	0	NULL	statement 1	Process		leads to		eventualy			senescence	Process				NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw60_molcellbiol_20_6_1947_s_19	10688642	For the yeast  Saccharomyces cerevisiae, genetic screens have identified five genes ( EST1,  EST2,  EST3,  EST4/CDC13, and  TLC1) ( 20,  27,  39) whose mutations lead to progressive telomere shortening and eventual loss of viability (i.e., senescence).	gene_phenotype
72181	3	334592	5	NULL	NULL	0	NULL	EST2 gene	GP	mutation of	leads to					telomere	Chromosome	progressive shortening of			NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw60_molcellbiol_20_6_1947_s_19	10688642	For the yeast  Saccharomyces cerevisiae, genetic screens have identified five genes ( EST1,  EST2,  EST3,  EST4/CDC13, and  TLC1) ( 20,  27,  39) whose mutations lead to progressive telomere shortening and eventual loss of viability (i.e., senescence).	gene_phenotype
72182	4	334592	5	NULL	NULL	0	NULL	statement 3	Process		leads to		eventualy			senescence	Process				NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw60_molcellbiol_20_6_1947_s_19	10688642	For the yeast  Saccharomyces cerevisiae, genetic screens have identified five genes ( EST1,  EST2,  EST3,  EST4/CDC13, and  TLC1) ( 20,  27,  39) whose mutations lead to progressive telomere shortening and eventual loss of viability (i.e., senescence).	gene_phenotype
72183	5	334592	5	NULL	NULL	0	NULL	EST3 gene	GP	mutation of	leads to					telomere	Chromosome	progressive shortening of			NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw60_molcellbiol_20_6_1947_s_19	10688642	For the yeast  Saccharomyces cerevisiae, genetic screens have identified five genes ( EST1,  EST2,  EST3,  EST4/CDC13, and  TLC1) ( 20,  27,  39) whose mutations lead to progressive telomere shortening and eventual loss of viability (i.e., senescence).	gene_phenotype
72184	6	334592	5	NULL	NULL	0	NULL	statement 5	Process		leads to		eventualy			senescence	Process				NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw60_molcellbiol_20_6_1947_s_19	10688642	For the yeast  Saccharomyces cerevisiae, genetic screens have identified five genes ( EST1,  EST2,  EST3,  EST4/CDC13, and  TLC1) ( 20,  27,  39) whose mutations lead to progressive telomere shortening and eventual loss of viability (i.e., senescence).	gene_phenotype
72185	7	334592	5	NULL	NULL	0	NULL	EST4/CDC13 gene	GP	mutation of	leads to					telomere	Chromosome	progressive shortening of			NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw60_molcellbiol_20_6_1947_s_19	10688642	For the yeast  Saccharomyces cerevisiae, genetic screens have identified five genes ( EST1,  EST2,  EST3,  EST4/CDC13, and  TLC1) ( 20,  27,  39) whose mutations lead to progressive telomere shortening and eventual loss of viability (i.e., senescence).	gene_phenotype
72186	8	334592	5	NULL	NULL	NULL	NULL	statement 7	Process		leads to		eventualy			senescence	Process				NULL	Saccharomyces cerevisiae	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_6_1947_s_19	10688642	For the yeast  Saccharomyces cerevisiae, genetic screens have identified five genes ( EST1,  EST2,  EST3,  EST4/CDC13, and  TLC1) ( 20,  27,  39) whose mutations lead to progressive telomere shortening and eventual loss of viability (i.e., senescence).	gene_phenotype
72187	9	334592	5	NULL	NULL	0	NULL	TLC1 gene	GP	mutation of	leads to					telomere	Chromosome	progressive shortening of			NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw60_molcellbiol_20_6_1947_s_19	10688642	For the yeast  Saccharomyces cerevisiae, genetic screens have identified five genes ( EST1,  EST2,  EST3,  EST4/CDC13, and  TLC1) ( 20,  27,  39) whose mutations lead to progressive telomere shortening and eventual loss of viability (i.e., senescence).	gene_phenotype
72188	10	334592	5	NULL	NULL	0	NULL	statement 9	Process		leads to		eventualy			senescence	Process				NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw60_molcellbiol_20_6_1947_s_19	10688642	For the yeast  Saccharomyces cerevisiae, genetic screens have identified five genes ( EST1,  EST2,  EST3,  EST4/CDC13, and  TLC1) ( 20,  27,  39) whose mutations lead to progressive telomere shortening and eventual loss of viability (i.e., senescence).	gene_phenotype
72189	1	334594	5	NULL	NULL	0	NULL	TLC1 gene	GP		encodes					telomerase	GP			RNA component	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_3_786_s_21	10629035	Yeast strains carrying a deletion of the  TLC1 gene, which encodes the RNA component of telomerase, show progressive telomere shortening, which ultimately leads to a loss of cell viability ( 53).	gene_phenotype
72190	2	334594	5	NULL	NULL	NULL	NULL	TLC1 gene	GP	deletion of	leads to					telomere	Chromosome	progressive shortening of			NULL	yeast strains	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_3_786_s_21	10629035	Yeast strains carrying a deletion of the  TLC1 gene, which encodes the RNA component of telomerase, show progressive telomere shortening, which ultimately leads to a loss of cell viability ( 53).	gene_phenotype
72191	3	334594	5	NULL	NULL	0	NULL	statement 2	Process		leads to		ultimately			cell viability	Process	loss of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_3_786_s_21	10629035	Yeast strains carrying a deletion of the  TLC1 gene, which encodes the RNA component of telomerase, show progressive telomere shortening, which ultimately leads to a loss of cell viability ( 53).	gene_phenotype
73579	1	334595	5	NULL	NULL	0	NULL	 yku80delta	GP	growth defect of;;mutant	is sensitive to					temperature	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_11_3721_s_15	12748277	Some of these components are interconnected; for instance, overexpression of the catalytic subunit of telomerase,  EST2, or of the telomerase RNA gene,  TLC1, suppressed the temperature-sensitive growth defect of a  yku80delta mutant at 37 degrees C ( 38,  49).	gene_phenotype
73580	2	334595	5	NULL	NULL	0	NULL	EST2	GP	overexpression of	suppress					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_11_3721_s_15	12748277	Some of these components are interconnected; for instance, overexpression of the catalytic subunit of telomerase,  EST2, or of the telomerase RNA gene,  TLC1, suppressed the temperature-sensitive growth defect of a  yku80delta mutant at 37 degrees C ( 38,  49).	gene_phenotype
73581	3	334595	5	NULL	NULL	NULL	NULL	TLC1 gene	GP	overexpression of	suppress					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_11_3721_s_15	12748277	Some of these components are interconnected; for instance, overexpression of the catalytic subunit of telomerase,  EST2, or of the telomerase RNA gene,  TLC1, suppressed the temperature-sensitive growth defect of a  yku80delta mutant at 37 degrees C ( 38,  49).	gene_phenotype
73582	4	334595	5	NULL	NULL	0	NULL	TLC1 gene	GP		is a type of					telomerase RNA gene	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_11_3721_s_15	12748277	Some of these components are interconnected; for instance, overexpression of the catalytic subunit of telomerase,  EST2, or of the telomerase RNA gene,  TLC1, suppressed the temperature-sensitive growth defect of a  yku80delta mutant at 37 degrees C ( 38,  49).	gene_phenotype
73583	5	334595	5	NULL	NULL	0	NULL	EST2	GP		is a subunit of		catalytic			telomerase	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_11_3721_s_15	12748277	Some of these components are interconnected; for instance, overexpression of the catalytic subunit of telomerase,  EST2, or of the telomerase RNA gene,  TLC1, suppressed the temperature-sensitive growth defect of a  yku80delta mutant at 37 degrees C ( 38,  49).	gene_phenotype
72257	1	334597	5	NULL	NULL	NULL	NULL	mtr10	GP		effects		specifically			Tlc1	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6046_s_301	12167699	The dispersed localization was not due to nuclear envelope leakiness, because the nucleolar RNA U3 had normal localization in  mtr10 cells (Fig.  6A), further suggesting a rather specific effect of  mtr10 on Tlc1.	gene_phenotype
72259	2	334597	5	NULL	NULL	0	NULL	RNA U3	NucleicAcid	nucleolar	is localized in		normal			mtr10 cells	Cell				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6046_s_301	12167699	The dispersed localization was not due to nuclear envelope leakiness, because the nucleolar RNA U3 had normal localization in  mtr10 cells (Fig.  6A), further suggesting a rather specific effect of  mtr10 on Tlc1.	gene_phenotype
72261	1	334598	5	NULL	NULL	0	NULL	telomere	Chromosome		is shortened in					mtr10 cells	Cell				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6046_s_308	12167699	This is the most likely cause of the telomere shortening observed in  mtr10 cells, because overexpression of  TLC1 in the mutant restored both telomere length and levels of mTlc1 without suppressing other aspects of the  mtr10 phenotype.	gene_phenotype
72263	2	334598	5	NULL	NULL	0	NULL	TLC1	NucleicAcid	overexpression of	restores					telomere	Chromosome	length of			NULL	mutant mtr10 cells	0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6046_s_308	12167699	This is the most likely cause of the telomere shortening observed in  mtr10 cells, because overexpression of  TLC1 in the mutant restored both telomere length and levels of mTlc1 without suppressing other aspects of the  mtr10 phenotype.	gene_phenotype
72264	3	334598	5	NULL	NULL	0	NULL	TLC1	NucleicAcid	overexpression of	restores					mTlc1	NucleicAcid	level of			NULL	mutant mtr10 cells	0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6046_s_308	12167699	This is the most likely cause of the telomere shortening observed in  mtr10 cells, because overexpression of  TLC1 in the mutant restored both telomere length and levels of mTlc1 without suppressing other aspects of the  mtr10 phenotype.	gene_phenotype
72265	1	334599	5	NULL	NULL	0	NULL	Est2p	GP		is a subunit of					telomerase	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_7_2182_s_254	11884605	It has been shown that overexpression of telomerase subunit Est2p or TLC1 suppresses checkpoint activation and restores viability at high temperature in Yku- cells without apparently modifying telomere length ( 75).	gene_phenotype
72266	2	334599	5	NULL	NULL	NULL	NULL	Est2p	GP	overexpression of	suppress					checkpoint	Process	activation of			NULL	Yku- cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_7_2182_s_254	11884605	It has been shown that overexpression of telomerase subunit Est2p or TLC1 suppresses checkpoint activation and restores viability at high temperature in Yku- cells without apparently modifying telomere length ( 75).	gene_phenotype
72267	3	334599	5	NULL	NULL	NULL	NULL	TLC1	NucleicAcid	overexpression of	suppress					checkpoint	Process	activation of			NULL	Yku- cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_7_2182_s_254	11884605	It has been shown that overexpression of telomerase subunit Est2p or TLC1 suppresses checkpoint activation and restores viability at high temperature in Yku- cells without apparently modifying telomere length ( 75).	gene_phenotype
72268	4	334599	5	NULL	NULL	0	NULL	statement 2	Process		restores					viability	Process				NULL	Yku- cells	0	NULL	NULL	NULL	gw60_molcellbiol_22_7_2182_s_254	11884605	It has been shown that overexpression of telomerase subunit Est2p or TLC1 suppresses checkpoint activation and restores viability at high temperature in Yku- cells without apparently modifying telomere length ( 75).	gene_phenotype
72269	5	334599	5	NULL	NULL	NULL	NULL	statement 4	Process		occurs without modifying					telomere	Chromosome	length of			NULL	Yku- cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_7_2182_s_254	11884605	It has been shown that overexpression of telomerase subunit Est2p or TLC1 suppresses checkpoint activation and restores viability at high temperature in Yku- cells without apparently modifying telomere length ( 75).	gene_phenotype
72270	6	334599	5	NULL	NULL	0	NULL	statement 3	Process		restores					viability	Process				NULL	Yku- cells	0	NULL	NULL	NULL	gw60_molcellbiol_22_7_2182_s_254	11884605	It has been shown that overexpression of telomerase subunit Est2p or TLC1 suppresses checkpoint activation and restores viability at high temperature in Yku- cells without apparently modifying telomere length ( 75).	gene_phenotype
72271	7	334599	5	NULL	NULL	NULL	NULL	statement 6	Process		occurs without modifying					telomere	Chromosome	length of			NULL	Yku- cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_22_7_2182_s_254	11884605	It has been shown that overexpression of telomerase subunit Est2p or TLC1 suppresses checkpoint activation and restores viability at high temperature in Yku- cells without apparently modifying telomere length ( 75).	gene_phenotype
72272	1	334600	5	NULL	NULL	0	NULL	TLC1 RNA	NucleicAcid	viable alleles of	is required for					telomere	Chromosome	function of			NULL	in vivo	0	NULL	NULL	NULL	gw60_molcellbiol_22_7_2366_s_3	11884619	A selection for viable alleles of  TLC1 RNA from a large library of random deletion alleles revealed that less than half ( 0.5 kb of the  1.3-kb RNA) is required for telomerase function in vivo.	gene_phenotype
72273	1	334601	5	NULL	NULL	NULL	NULL	telomerase	GP	yeast	is encoded by				RNA subunit	TLC1 gene	GP	yeast			NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_17_9202_s_23	9256460	Although the RNA subunit of yeast telomerase is known to be encoded by the gene  TLC1 ( 20) and is essential for telomerase catalysis ( 19), no yeast protein has heretofore been found to be essential for telomerase enzyme activity.	gene_phenotype
72274	2	334601	5	NULL	NULL	0	NULL	TLC1 gene	GP	yeast	is essential for					telomerase	GP	catalysis of			NULL		0	NULL	NULL	NULL	gw60_pnas_94_17_9202_s_23	9256460	Although the RNA subunit of yeast telomerase is known to be encoded by the gene  TLC1 ( 20) and is essential for telomerase catalysis ( 19), no yeast protein has heretofore been found to be essential for telomerase enzyme activity.	gene_phenotype
72275	1	334602	5	NULL	NULL	0	NULL	TLC1	NucleicAcid	mutant	decreases		gradually			telomere	Chromosome	length of			NULL		0	NULL	NULL	NULL	gw60_pnas_94_17_9202_s_24	9256460	TLC1 mutants ( 20) exhibit two phenotypes that are shared by mutants of the genes  EST1 ( 21) and  CDC13 ( 22-24): a gradual decrease in telomere length and a consequent decline in cell viability.	gene_phenotype
72276	2	334602	5	NULL	NULL	0	NULL	statement 1	Process		decline		consequently			cell viability	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_94_17_9202_s_24	9256460	TLC1 mutants ( 20) exhibit two phenotypes that are shared by mutants of the genes  EST1 ( 21) and  CDC13 ( 22-24): a gradual decrease in telomere length and a consequent decline in cell viability.	gene_phenotype
72277	3	334602	5	NULL	NULL	0	NULL	EST1 gene	GP	mutant	decreases		gradually			telomere	Chromosome	length of			NULL		0	NULL	NULL	NULL	gw60_pnas_94_17_9202_s_24	9256460	TLC1 mutants ( 20) exhibit two phenotypes that are shared by mutants of the genes  EST1 ( 21) and  CDC13 ( 22-24): a gradual decrease in telomere length and a consequent decline in cell viability.	gene_phenotype
72278	4	334602	5	NULL	NULL	NULL	NULL	statement 3	Process		decline		consequently			cell viability	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_17_9202_s_24	9256460	TLC1 mutants ( 20) exhibit two phenotypes that are shared by mutants of the genes  EST1 ( 21) and  CDC13 ( 22-24): a gradual decrease in telomere length and a consequent decline in cell viability.	gene_phenotype
72279	5	334602	5	NULL	NULL	0	NULL	CDC13 gene	GP	mutant	decreases		gradually			telomere	Chromosome	length of			NULL		0	NULL	NULL	NULL	gw60_pnas_94_17_9202_s_24	9256460	TLC1 mutants ( 20) exhibit two phenotypes that are shared by mutants of the genes  EST1 ( 21) and  CDC13 ( 22-24): a gradual decrease in telomere length and a consequent decline in cell viability.	gene_phenotype
72280	6	334602	5	NULL	NULL	0	NULL	statement 5	Process		decreases		consequently			cell viability	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_94_17_9202_s_24	9256460	TLC1 mutants ( 20) exhibit two phenotypes that are shared by mutants of the genes  EST1 ( 21) and  CDC13 ( 22-24): a gradual decrease in telomere length and a consequent decline in cell viability.	gene_phenotype
72281	1	334603	5	NULL	NULL	0	NULL	tTLC1	NucleicAcid		is					dominant truncated allele of TLC1	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_pnas_94_18_9768_s_57	9275199	Thus, we overexpressed the dominant truncated allele of  TLC1 ( tTLC1), which was shown to result in telomeres adopting a shorter steady-state length (ref.  9; Fig.  1 A, lane 3).	gene_phenotype
72282	3	334603	5	NULL	NULL	0	NULL	tTLC1	NucleicAcid		results in					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_94_18_9768_s_57	9275199	Thus, we overexpressed the dominant truncated allele of  TLC1 ( tTLC1), which was shown to result in telomeres adopting a shorter steady-state length (ref.  9; Fig.  1 A, lane 3).	gene_phenotype
72283	2	334603	5	NULL	NULL	0	NULL	telomere	Chromosome		adopt					steady-state length	PhysicalPhenomenon	short			NULL		0	NULL	NULL	NULL	gw60_pnas_94_18_9768_s_57	9275199	Thus, we overexpressed the dominant truncated allele of  TLC1 ( tTLC1), which was shown to result in telomeres adopting a shorter steady-state length (ref.  9; Fig.  1 A, lane 3).	gene_phenotype
72284	1	334604	5	NULL	NULL	0	NULL	telomere 	Chromosome	length of	is inversly related to					lifespan	Time				NULL		0	NULL	NULL	NULL	gw60_pnas_94_18_9768_s_87	9275199	While the above experiments suggested that telomere length was inversely related to lifespan, it was possible that the mutations in  TLC1 or  RAP1 used to alter telomere length affected lifespan in some other way.	gene_phenotype
72285	2	334604	5	NULL	NULL	0	NULL	TLC1	NucleicAcid	mutation of	alter					telomere	Chromosome	length of			NULL		0	NULL	NULL	NULL	gw60_pnas_94_18_9768_s_87	9275199	While the above experiments suggested that telomere length was inversely related to lifespan, it was possible that the mutations in  TLC1 or  RAP1 used to alter telomere length affected lifespan in some other way.	gene_phenotype
72286	3	334604	5	NULL	NULL	0	NULL	statement 2	Process		affects		possibly			lifespan	Time				NULL		0	NULL	NULL	NULL	gw60_pnas_94_18_9768_s_87	9275199	While the above experiments suggested that telomere length was inversely related to lifespan, it was possible that the mutations in  TLC1 or  RAP1 used to alter telomere length affected lifespan in some other way.	gene_phenotype
72287	4	334604	5	NULL	NULL	0	NULL	RAP1	GP	mutation of	alter					telomere	Chromosome	length of			NULL		0	NULL	NULL	NULL	gw60_pnas_94_18_9768_s_87	9275199	While the above experiments suggested that telomere length was inversely related to lifespan, it was possible that the mutations in  TLC1 or  RAP1 used to alter telomere length affected lifespan in some other way.	gene_phenotype
72288	5	334604	5	NULL	NULL	0	NULL	statement 4	Process		affects		possibly			lifespan	Time				NULL		0	NULL	NULL	NULL	gw60_pnas_94_18_9768_s_87	9275199	While the above experiments suggested that telomere length was inversely related to lifespan, it was possible that the mutations in  TLC1 or  RAP1 used to alter telomere length affected lifespan in some other way.	gene_phenotype
72290	1	334605	5	NULL	NULL	0	NULL	rad50	GP	mutant	resistant to					ionizing radiation	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	abs-batch0550-0559_genetics_160_1_11805044_s_4	11805044	Overexpression of EXO1 or TLC1 increased the resistance of rad50,  mre11, and xrs2 mutants to ionizing radiation and MMS, but did not increase  resistance in strains defective in recombination (rad51, rad52, rad54,  rad59) or NHEJ only (yku70, sir4).	gene_phenotype
72291	2	334605	5	NULL	NULL	0	NULL	mre11	GP	mutant	resistant to					ionizing radiation	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	abs-batch0550-0559_genetics_160_1_11805044_s_4	11805044	Overexpression of EXO1 or TLC1 increased the resistance of rad50,  mre11, and xrs2 mutants to ionizing radiation and MMS, but did not increase  resistance in strains defective in recombination (rad51, rad52, rad54,  rad59) or NHEJ only (yku70, sir4).	gene_phenotype
72292	3	334605	5	NULL	NULL	0	NULL	xrs2	GP	mutant	resistant to					ionizing radiation	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	abs-batch0550-0559_genetics_160_1_11805044_s_4	11805044	Overexpression of EXO1 or TLC1 increased the resistance of rad50,  mre11, and xrs2 mutants to ionizing radiation and MMS, but did not increase  resistance in strains defective in recombination (rad51, rad52, rad54,  rad59) or NHEJ only (yku70, sir4).	gene_phenotype
72293	4	334605	5	NULL	NULL	0	NULL	rad50	GP	mutant	resistant to					MMS	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0550-0559_genetics_160_1_11805044_s_4	11805044	Overexpression of EXO1 or TLC1 increased the resistance of rad50,  mre11, and xrs2 mutants to ionizing radiation and MMS, but did not increase  resistance in strains defective in recombination (rad51, rad52, rad54,  rad59) or NHEJ only (yku70, sir4).	gene_phenotype
72295	5	334605	5	NULL	NULL	0	NULL	mre11	GP	mutant	resistant to					MMS	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0550-0559_genetics_160_1_11805044_s_4	11805044	Overexpression of EXO1 or TLC1 increased the resistance of rad50,  mre11, and xrs2 mutants to ionizing radiation and MMS, but did not increase  resistance in strains defective in recombination (rad51, rad52, rad54,  rad59) or NHEJ only (yku70, sir4).	gene_phenotype
72296	6	334605	5	NULL	NULL	0	NULL	xrs2	GP	mutant	resistant to					MMS	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0550-0559_genetics_160_1_11805044_s_4	11805044	Overexpression of EXO1 or TLC1 increased the resistance of rad50,  mre11, and xrs2 mutants to ionizing radiation and MMS, but did not increase  resistance in strains defective in recombination (rad51, rad52, rad54,  rad59) or NHEJ only (yku70, sir4).	gene_phenotype
72298	7	334605	5	NULL	NULL	0	NULL	EXO1	GP	overexpression of	increases					statement 1	Process				NULL		0	NULL	NULL	NULL	abs-batch0550-0559_genetics_160_1_11805044_s_4	11805044	Overexpression of EXO1 or TLC1 increased the resistance of rad50,  mre11, and xrs2 mutants to ionizing radiation and MMS, but did not increase  resistance in strains defective in recombination (rad51, rad52, rad54,  rad59) or NHEJ only (yku70, sir4).	gene_phenotype
72299	8	334605	5	NULL	NULL	0	NULL	EXO1	GP	overexpression of	increases					statement 2	Process				NULL		0	NULL	NULL	NULL	abs-batch0550-0559_genetics_160_1_11805044_s_4	11805044	Overexpression of EXO1 or TLC1 increased the resistance of rad50,  mre11, and xrs2 mutants to ionizing radiation and MMS, but did not increase  resistance in strains defective in recombination (rad51, rad52, rad54,  rad59) or NHEJ only (yku70, sir4).	gene_phenotype
72300	1	334607	5	NULL	NULL	0	NULL	TLC1 RNA	NucleicAcid	viable alleles of	is required for					telomerase	GP	function of			NULL	in vivo	0	NULL	NULL	NULL	abs-batch0650-0679_mol-cell-biol_22_7_11884619_s_3	11884619	A selection for viable alleles of TLC1 RNA from a large library  of random deletion alleles revealed that less than half (approximately  0.5 kb of the approximately 1.3-kb RNA) is required for telomerase function  in vivo.	gene_phenotype
72301	1	334608	5	NULL	NULL	0	NULL	EST2	GP	overexpression of	does not restore					DNA repair	Process	efficient			NULL	yku80 mutants	0	NULL	NULL	NULL	abs-batch0650-0679_embo-rep_2_3_11266360_s_5	11266360	We show that overexpression of EST2 or TLC1 in  yku80 mutants does not restore efficient DNA repair, or restore normal  telomere function, as measured by telomere length, single-stranded G-rich  strand or transcriptional silencing.	gene_phenotype
72302	2	334608	5	NULL	NULL	0	NULL	TLC1	NucleicAcid	overexpression of	does not restore					DNA repair	Process	efficient			NULL	yku80 mutants	0	NULL	NULL	NULL	abs-batch0650-0679_embo-rep_2_3_11266360_s_5	11266360	We show that overexpression of EST2 or TLC1 in  yku80 mutants does not restore efficient DNA repair, or restore normal  telomere function, as measured by telomere length, single-stranded G-rich  strand or transcriptional silencing.	gene_phenotype
72303	3	334608	5	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_embo-rep_2_3_11266360_s_5	11266360	We show that overexpression of EST2 or TLC1 in  yku80 mutants does not restore efficient DNA repair, or restore normal  telomere function, as measured by telomere length, single-stranded G-rich  strand or transcriptional silencing.	gene_phenotype
72306	4	334608	5	NULL	NULL	0	NULL	EST2	GP	overexpression of	does not restore					telomere	Chromosome	normal function of			NULL	yku80 mutants	0	NULL	NULL	NULL	abs-batch0650-0679_embo-rep_2_3_11266360_s_5	11266360	We show that overexpression of EST2 or TLC1 in  yku80 mutants does not restore efficient DNA repair, or restore normal  telomere function, as measured by telomere length, single-stranded G-rich  strand or transcriptional silencing.	gene_phenotype
72307	5	334608	5	NULL	NULL	0	NULL	TLC1	NucleicAcid	overexpression of	does not restore					telomere	Chromosome	normal function of			NULL	yku80 mutants	0	NULL	NULL	NULL	abs-batch0650-0679_embo-rep_2_3_11266360_s_5	11266360	We show that overexpression of EST2 or TLC1 in  yku80 mutants does not restore efficient DNA repair, or restore normal  telomere function, as measured by telomere length, single-stranded G-rich  strand or transcriptional silencing.	gene_phenotype
72308	6	334608	5	NULL	NULL	0	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_embo-rep_2_3_11266360_s_5	11266360	We show that overexpression of EST2 or TLC1 in  yku80 mutants does not restore efficient DNA repair, or restore normal  telomere function, as measured by telomere length, single-stranded G-rich  strand or transcriptional silencing.	gene_phenotype
72319	1	334610	5	NULL	NULL	0	NULL	telomeric circle-mediated targeting	Process		occurs in		frequently			type I tlc1 survivors	Cell	established			NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_4_2_327_s_215	15701795	In addition, established type I and type II  tlc1 survivors both displayed a 20% higher frequency in telomeric circle-mediated targeting than the  tlc1 cells right from sporulation and prior to the survivor formation (Table  1), suggesting that telomeric circle-mediated targeting occurs more frequently in established type I and type II survivors.	gene_phenotype
72320	2	334610	5	NULL	NULL	NULL	NULL	telomeric circle-mediated targeting	Process		occurs in		frequently			type II tlc1 survivors	Cell	established			NULL		NULL	NULL	NULL	NULL	gw70_eukaryotcell_4_2_327_s_215	15701795	In addition, established type I and type II  tlc1 survivors both displayed a 20% higher frequency in telomeric circle-mediated targeting than the  tlc1 cells right from sporulation and prior to the survivor formation (Table  1), suggesting that telomeric circle-mediated targeting occurs more frequently in established type I and type II survivors.	gene_phenotype
72327	2	334611	5	NULL	NULL	NULL	NULL	telomere	Chromosome	defect in	leads to		probably			tlc1-h tlc1-h homozygote 	Cell	poor sporulation efficiency of 			NULL		NULL	NULL	NULL	NULL	gw70_embo_22_7_1697_s_120	12660175	Since the sporulation efficiency of  tlc1-h tlc1-h homozygote was very poor, probably due to their telomeric defects, the production  of mutated haploid cells from the diploids was very inefficient.	gene_phenotype
72329	1	334611	5	NULL	NULL	0	NULL	haploid cells	Cell		is produced from					diploids	Cell				NULL		0	NULL	NULL	NULL	gw70_embo_22_7_1697_s_120	12660175	Since the sporulation efficiency of  tlc1-h tlc1-h homozygote was very poor, probably due to their telomeric defects, the production  of mutated haploid cells from the diploids was very inefficient.	gene_phenotype
72330	3	334611	5	NULL	NULL	0	NULL	statement 2	Process		leads to					statement 1	Process	inefficient;;mutant			NULL		0	NULL	NULL	NULL	gw70_embo_22_7_1697_s_120	12660175	Since the sporulation efficiency of  tlc1-h tlc1-h homozygote was very poor, probably due to their telomeric defects, the production  of mutated haploid cells from the diploids was very inefficient.	gene_phenotype
72331	1	334613	5	NULL	NULL	NULL	NULL	Rap1p	GP		is absent in					VII-L telomere	Chromosome				NULL		NULL	NULL	NULL	NULL	gw70_embo_22_7_1688_s_219	12660174	Since the YH/YH diploid, with its mixture of yeast and vertebrate telomeric DNA  at all telomeres, was as defective in meiosis as the H/H strain that was homozygous  for the C3TA2 telomere ( Figure 4B), the meiotic defect of the  tlc1h strain can not be attributed solely to the absence of Rap1p at the VII-L telomere.	gene_phenotype
72332	2	334613	5	NULL	NULL	0	NULL	tlc1h strain	Cell	meiotic defect of 	is not attributed to		solely			statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_embo_22_7_1688_s_219	12660174	Since the YH/YH diploid, with its mixture of yeast and vertebrate telomeric DNA  at all telomeres, was as defective in meiosis as the H/H strain that was homozygous  for the C3TA2 telomere ( Figure 4B), the meiotic defect of the  tlc1h strain can not be attributed solely to the absence of Rap1p at the VII-L telomere.	gene_phenotype
72333	3	334613	5	NULL	NULL	0	NULL	YH/YH diploid	Cell		contains					telomeric DNA	NucleicAcid	mixture of;;yeast and vertebrate			NULL	telomeres	0	NULL	NULL	NULL	gw70_embo_22_7_1688_s_219	12660174	Since the YH/YH diploid, with its mixture of yeast and vertebrate telomeric DNA  at all telomeres, was as defective in meiosis as the H/H strain that was homozygous  for the C3TA2 telomere ( Figure 4B), the meiotic defect of the  tlc1h strain can not be attributed solely to the absence of Rap1p at the VII-L telomere.	gene_phenotype
72334	4	334613	5	NULL	NULL	0	NULL	statement 3	Cell		is defective in					meiosis	Process				NULL		0	NULL	NULL	NULL	gw70_embo_22_7_1688_s_219	12660174	Since the YH/YH diploid, with its mixture of yeast and vertebrate telomeric DNA  at all telomeres, was as defective in meiosis as the H/H strain that was homozygous  for the C3TA2 telomere ( Figure 4B), the meiotic defect of the  tlc1h strain can not be attributed solely to the absence of Rap1p at the VII-L telomere.	gene_phenotype
72335	5	334613	5	NULL	NULL	0	NULL	H/H strain	Cell		is homozygous for					C3TA2 telomere	Chromosome				NULL		0	NULL	NULL	NULL	gw70_embo_22_7_1688_s_219	12660174	Since the YH/YH diploid, with its mixture of yeast and vertebrate telomeric DNA  at all telomeres, was as defective in meiosis as the H/H strain that was homozygous  for the C3TA2 telomere ( Figure 4B), the meiotic defect of the  tlc1h strain can not be attributed solely to the absence of Rap1p at the VII-L telomere.	gene_phenotype
72336	6	334613	5	NULL	NULL	0	NULL	statement 5	Cell		is defective in					meiosis	Process				NULL		0	NULL	NULL	NULL	gw70_embo_22_7_1688_s_219	12660174	Since the YH/YH diploid, with its mixture of yeast and vertebrate telomeric DNA  at all telomeres, was as defective in meiosis as the H/H strain that was homozygous  for the C3TA2 telomere ( Figure 4B), the meiotic defect of the  tlc1h strain can not be attributed solely to the absence of Rap1p at the VII-L telomere.	gene_phenotype
72337	1	334614	5	NULL	NULL	0	NULL	TLC1	NucleicAcid	full-length	disrupts					telomeric silencing	Process				NULL		0	NULL	NULL	NULL	gw70_genesdev_17_19_2384_s_47	12975323	The triple stem-loop had been found previously to most closely match the activity of full-length TLC1 in disrupting telomeric silencing (Peterson et al. 2001 ), perhaps because the stem-loop can fold most stably in this construct.	gene_phenotype
72338	2	334614	5	NULL	NULL	0	NULL	triple stem-loop	NucleicAcid		disrupts					telomeric silencing	Process				NULL		0	NULL	NULL	NULL	gw70_genesdev_17_19_2384_s_47	12975323	The triple stem-loop had been found previously to most closely match the activity of full-length TLC1 in disrupting telomeric silencing (Peterson et al. 2001 ), perhaps because the stem-loop can fold most stably in this construct.	gene_phenotype
72339	1	334615	5	NULL	NULL	0	NULL	Ku	GP		bind					TLC1 RNA	NucleicAcid			stem-loop	NULL		0	NULL	NULL	NULL	gw70_genesdev_17_19_2384_s_156	12975323	It disrupts Ku's ability to bind the 48-nucleotide stem-loop of TLC1 RNA, but retains Ku's ability to bind DNA, as well as many of Ku's DNA-based activities, namely telomeric silencing, chromosome end protection, and DNA repair via NHEJ.	gene_phenotype
72340	2	334615	5	NULL	NULL	0	NULL	Ku	GP		bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_genesdev_17_19_2384_s_156	12975323	It disrupts Ku's ability to bind the 48-nucleotide stem-loop of TLC1 RNA, but retains Ku's ability to bind DNA, as well as many of Ku's DNA-based activities, namely telomeric silencing, chromosome end protection, and DNA repair via NHEJ.	gene_phenotype
72341	3	334615	5	NULL	NULL	0	NULL	Ku	GP		activates					telomeric silencing	Process				NULL		0	NULL	NULL	NULL	gw70_genesdev_17_19_2384_s_156	12975323	It disrupts Ku's ability to bind the 48-nucleotide stem-loop of TLC1 RNA, but retains Ku's ability to bind DNA, as well as many of Ku's DNA-based activities, namely telomeric silencing, chromosome end protection, and DNA repair via NHEJ.	gene_phenotype
72342	4	334615	5	NULL	NULL	0	NULL	Ku	GP		activates					chromosome end 	Chromosome	protection of			NULL		0	NULL	NULL	NULL	gw70_genesdev_17_19_2384_s_156	12975323	It disrupts Ku's ability to bind the 48-nucleotide stem-loop of TLC1 RNA, but retains Ku's ability to bind DNA, as well as many of Ku's DNA-based activities, namely telomeric silencing, chromosome end protection, and DNA repair via NHEJ.	gene_phenotype
72343	5	334615	5	NULL	NULL	0	NULL	Ku	GP		activates					DNA	NucleicAcid	repair of			NULL		0	NULL	NULL	NULL	gw70_genesdev_17_19_2384_s_156	12975323	It disrupts Ku's ability to bind the 48-nucleotide stem-loop of TLC1 RNA, but retains Ku's ability to bind DNA, as well as many of Ku's DNA-based activities, namely telomeric silencing, chromosome end protection, and DNA repair via NHEJ.	gene_phenotype
72344	6	334615	5	NULL	NULL	0	NULL	statement 5	Process		via					NHEJ	Process				NULL		0	NULL	NULL	NULL	gw70_genesdev_17_19_2384_s_156	12975323	It disrupts Ku's ability to bind the 48-nucleotide stem-loop of TLC1 RNA, but retains Ku's ability to bind DNA, as well as many of Ku's DNA-based activities, namely telomeric silencing, chromosome end protection, and DNA repair via NHEJ.	gene_phenotype
72345	1	334616	5	NULL	NULL	0	NULL	telomerase activity	Process		is dependent on					Est2p activity	Process	Saccharomyces cerevisiae			NULL	in vitro	0	NULL	NULL	NULL	gw70_genesdev_18_15_1781_s_21	15289453	Although in vitro telomerase activity is dependent on the activity of the reverse transcriptase catalytic subunit (Est2p in the budding yeast  Saccharomyces cerevisiae; TERT in mammals) and the telomerase RNA template (Tlc1 in  S. cerevisiae and hTR in humans), other factors are clearly needed for telomerase action in vivo (see  Table 1).	gene_phenotype
72346	2	334616	5	NULL	NULL	0	NULL	telomerase activity	Process		is dependent on					TERT activity	Process	mammals			NULL	in vitro	0	NULL	NULL	NULL	gw70_genesdev_18_15_1781_s_21	15289453	Although in vitro telomerase activity is dependent on the activity of the reverse transcriptase catalytic subunit (Est2p in the budding yeast  Saccharomyces cerevisiae; TERT in mammals) and the telomerase RNA template (Tlc1 in  S. cerevisiae and hTR in humans), other factors are clearly needed for telomerase action in vivo (see  Table 1).	gene_phenotype
72347	3	334616	5	NULL	NULL	0	NULL	telomerase activity	Process		is dependent on					Tlc1	NucleicAcid	S.cerevisiae			NULL	in vitro	0	NULL	NULL	NULL	gw70_genesdev_18_15_1781_s_21	15289453	Although in vitro telomerase activity is dependent on the activity of the reverse transcriptase catalytic subunit (Est2p in the budding yeast  Saccharomyces cerevisiae; TERT in mammals) and the telomerase RNA template (Tlc1 in  S. cerevisiae and hTR in humans), other factors are clearly needed for telomerase action in vivo (see  Table 1).	gene_phenotype
72348	4	334616	5	NULL	NULL	NULL	NULL	telomerase activity	Process		is dependent on					hTR	NucleicAcid	human			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_genesdev_18_15_1781_s_21	15289453	Although in vitro telomerase activity is dependent on the activity of the reverse transcriptase catalytic subunit (Est2p in the budding yeast  Saccharomyces cerevisiae; TERT in mammals) and the telomerase RNA template (Tlc1 in  S. cerevisiae and hTR in humans), other factors are clearly needed for telomerase action in vivo (see  Table 1).	gene_phenotype
72349	5	334616	5	NULL	NULL	0	NULL	Est2p	GP	Saccharomyces cerevisiae	is a subunit of		catalytic			reverse transcriptase	GP	Saccharomyces cerevisiae			NULL		0	NULL	NULL	NULL	gw70_genesdev_18_15_1781_s_21	15289453	Although in vitro telomerase activity is dependent on the activity of the reverse transcriptase catalytic subunit (Est2p in the budding yeast  Saccharomyces cerevisiae; TERT in mammals) and the telomerase RNA template (Tlc1 in  S. cerevisiae and hTR in humans), other factors are clearly needed for telomerase action in vivo (see  Table 1).	gene_phenotype
72350	6	334616	5	NULL	NULL	0	NULL	TERT	GP	mammals	is a subunit of		catalytic			reverse transcriptase	GP	mammals			NULL		0	NULL	NULL	NULL	gw70_genesdev_18_15_1781_s_21	15289453	Although in vitro telomerase activity is dependent on the activity of the reverse transcriptase catalytic subunit (Est2p in the budding yeast  Saccharomyces cerevisiae; TERT in mammals) and the telomerase RNA template (Tlc1 in  S. cerevisiae and hTR in humans), other factors are clearly needed for telomerase action in vivo (see  Table 1).	gene_phenotype
72351	7	334616	5	NULL	NULL	0	NULL	Tlc1	NucleicAcid	S. cerevisiae	is a type of					telomerase RNA template	NucleicAcid	S.cerevisiae			NULL		0	NULL	NULL	NULL	gw70_genesdev_18_15_1781_s_21	15289453	Although in vitro telomerase activity is dependent on the activity of the reverse transcriptase catalytic subunit (Est2p in the budding yeast  Saccharomyces cerevisiae; TERT in mammals) and the telomerase RNA template (Tlc1 in  S. cerevisiae and hTR in humans), other factors are clearly needed for telomerase action in vivo (see  Table 1).	gene_phenotype
72352	8	334616	5	NULL	NULL	0	NULL	hTR	NucleicAcid	human	is a type of					telomerase RNA template	NucleicAcid	human			NULL		0	NULL	NULL	NULL	gw70_genesdev_18_15_1781_s_21	15289453	Although in vitro telomerase activity is dependent on the activity of the reverse transcriptase catalytic subunit (Est2p in the budding yeast  Saccharomyces cerevisiae; TERT in mammals) and the telomerase RNA template (Tlc1 in  S. cerevisiae and hTR in humans), other factors are clearly needed for telomerase action in vivo (see  Table 1).	gene_phenotype
72381	1	334619	5	NULL	NULL	0	NULL	repetitive sequences	NucleicAcid		is maintained by					telomerase	GP				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_177_s_14	15189140	Telomeres are composed of repetitive sequences that can be maintained  by telomerase, a complex containing a reverse transcriptase (hTERT in humans and  Est2 in budding yeast), a template RNA (hTERC in humans and Tlc1 in yeast), and accessory  factors (the Est1 proteins and dyskerin in humans and Est1, Est3, and Sm proteins  in budding yeast).	gene_phenotype
72382	2	334619	5	NULL	NULL	0	NULL	telomeres	Chromosome		is composed of					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_177_s_14	15189140	Telomeres are composed of repetitive sequences that can be maintained  by telomerase, a complex containing a reverse transcriptase (hTERT in humans and  Est2 in budding yeast), a template RNA (hTERC in humans and Tlc1 in yeast), and accessory  factors (the Est1 proteins and dyskerin in humans and Est1, Est3, and Sm proteins  in budding yeast).	gene_phenotype
72383	3	334619	5	NULL	NULL	NULL	NULL	telomerase	GP		is a complex of					hTERT	GP				NULL	human	NULL	NULL	NULL	NULL	gw70_annurevbiochem_73_0_177_s_14	15189140	Telomeres are composed of repetitive sequences that can be maintained  by telomerase, a complex containing a reverse transcriptase (hTERT in humans and  Est2 in budding yeast), a template RNA (hTERC in humans and Tlc1 in yeast), and accessory  factors (the Est1 proteins and dyskerin in humans and Est1, Est3, and Sm proteins  in budding yeast).	gene_phenotype
72384	4	334619	5	NULL	NULL	0	NULL	telomerase	GP		is a complex of					hTERC	NucleicAcid				NULL	human	0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_177_s_14	15189140	Telomeres are composed of repetitive sequences that can be maintained  by telomerase, a complex containing a reverse transcriptase (hTERT in humans and  Est2 in budding yeast), a template RNA (hTERC in humans and Tlc1 in yeast), and accessory  factors (the Est1 proteins and dyskerin in humans and Est1, Est3, and Sm proteins  in budding yeast).	gene_phenotype
72385	5	334619	5	NULL	NULL	0	NULL	telomerase	GP		is a complex of					Est1 protein	GP				NULL	human	0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_177_s_14	15189140	Telomeres are composed of repetitive sequences that can be maintained  by telomerase, a complex containing a reverse transcriptase (hTERT in humans and  Est2 in budding yeast), a template RNA (hTERC in humans and Tlc1 in yeast), and accessory  factors (the Est1 proteins and dyskerin in humans and Est1, Est3, and Sm proteins  in budding yeast).	gene_phenotype
72386	6	334619	5	NULL	NULL	0	NULL	telomerase	GP		is a complex of					dyskerin	GP				NULL	human	0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_177_s_14	15189140	Telomeres are composed of repetitive sequences that can be maintained  by telomerase, a complex containing a reverse transcriptase (hTERT in humans and  Est2 in budding yeast), a template RNA (hTERC in humans and Tlc1 in yeast), and accessory  factors (the Est1 proteins and dyskerin in humans and Est1, Est3, and Sm proteins  in budding yeast).	gene_phenotype
72387	7	334619	5	NULL	NULL	0	NULL	statement 3	Process		occurs along with					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_177_s_14	15189140	Telomeres are composed of repetitive sequences that can be maintained  by telomerase, a complex containing a reverse transcriptase (hTERT in humans and  Est2 in budding yeast), a template RNA (hTERC in humans and Tlc1 in yeast), and accessory  factors (the Est1 proteins and dyskerin in humans and Est1, Est3, and Sm proteins  in budding yeast).	gene_phenotype
72388	8	334619	5	NULL	NULL	0	NULL	statement 5	Process		occurs along with					statement 6	Process				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_177_s_14	15189140	Telomeres are composed of repetitive sequences that can be maintained  by telomerase, a complex containing a reverse transcriptase (hTERT in humans and  Est2 in budding yeast), a template RNA (hTERC in humans and Tlc1 in yeast), and accessory  factors (the Est1 proteins and dyskerin in humans and Est1, Est3, and Sm proteins  in budding yeast).	gene_phenotype
72389	9	334619	5	NULL	NULL	0	NULL	statement 7	Process		occurs along with					statement 8	Process				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_177_s_14	15189140	Telomeres are composed of repetitive sequences that can be maintained  by telomerase, a complex containing a reverse transcriptase (hTERT in humans and  Est2 in budding yeast), a template RNA (hTERC in humans and Tlc1 in yeast), and accessory  factors (the Est1 proteins and dyskerin in humans and Est1, Est3, and Sm proteins  in budding yeast).	gene_phenotype
72390	10	334619	5	NULL	NULL	0	NULL	telomerase	GP		is a complex of					Est2	GP				NULL	budding yeast	0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_177_s_14	15189140	Telomeres are composed of repetitive sequences that can be maintained  by telomerase, a complex containing a reverse transcriptase (hTERT in humans and  Est2 in budding yeast), a template RNA (hTERC in humans and Tlc1 in yeast), and accessory  factors (the Est1 proteins and dyskerin in humans and Est1, Est3, and Sm proteins  in budding yeast).	gene_phenotype
72391	11	334619	5	NULL	NULL	0	NULL	telomerase	GP		is a complex of					Tlc1	NucleicAcid				NULL	budding yeast	0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_177_s_14	15189140	Telomeres are composed of repetitive sequences that can be maintained  by telomerase, a complex containing a reverse transcriptase (hTERT in humans and  Est2 in budding yeast), a template RNA (hTERC in humans and Tlc1 in yeast), and accessory  factors (the Est1 proteins and dyskerin in humans and Est1, Est3, and Sm proteins  in budding yeast).	gene_phenotype
72392	12	334619	5	NULL	NULL	0	NULL	telomerase	GP		is a complex of					Est1 protein	GP				NULL	budding yeast	0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_177_s_14	15189140	Telomeres are composed of repetitive sequences that can be maintained  by telomerase, a complex containing a reverse transcriptase (hTERT in humans and  Est2 in budding yeast), a template RNA (hTERC in humans and Tlc1 in yeast), and accessory  factors (the Est1 proteins and dyskerin in humans and Est1, Est3, and Sm proteins  in budding yeast).	gene_phenotype
72393	13	334619	5	NULL	NULL	0	NULL	telomerase	GP		is a complex of					Est3 protein	GP				NULL	budding yeast	0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_177_s_14	15189140	Telomeres are composed of repetitive sequences that can be maintained  by telomerase, a complex containing a reverse transcriptase (hTERT in humans and  Est2 in budding yeast), a template RNA (hTERC in humans and Tlc1 in yeast), and accessory  factors (the Est1 proteins and dyskerin in humans and Est1, Est3, and Sm proteins  in budding yeast).	gene_phenotype
72394	14	334619	5	NULL	NULL	0	NULL	telomerase	GP		is a complex of					Sm protein	GP				NULL	budding yeast	0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_177_s_14	15189140	Telomeres are composed of repetitive sequences that can be maintained  by telomerase, a complex containing a reverse transcriptase (hTERT in humans and  Est2 in budding yeast), a template RNA (hTERC in humans and Tlc1 in yeast), and accessory  factors (the Est1 proteins and dyskerin in humans and Est1, Est3, and Sm proteins  in budding yeast).	gene_phenotype
72395	15	334619	5	NULL	NULL	0	NULL	statement 10	Process		occurs along with					statement 11	Process				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_177_s_14	15189140	Telomeres are composed of repetitive sequences that can be maintained  by telomerase, a complex containing a reverse transcriptase (hTERT in humans and  Est2 in budding yeast), a template RNA (hTERC in humans and Tlc1 in yeast), and accessory  factors (the Est1 proteins and dyskerin in humans and Est1, Est3, and Sm proteins  in budding yeast).	gene_phenotype
72396	16	334619	5	NULL	NULL	0	NULL	statement 12	Process		occurs along with					statement 13	Process				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_177_s_14	15189140	Telomeres are composed of repetitive sequences that can be maintained  by telomerase, a complex containing a reverse transcriptase (hTERT in humans and  Est2 in budding yeast), a template RNA (hTERC in humans and Tlc1 in yeast), and accessory  factors (the Est1 proteins and dyskerin in humans and Est1, Est3, and Sm proteins  in budding yeast).	gene_phenotype
72397	17	334619	5	NULL	NULL	0	NULL	statement 15	Process		occurs along with					statement 16	Process				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_177_s_14	15189140	Telomeres are composed of repetitive sequences that can be maintained  by telomerase, a complex containing a reverse transcriptase (hTERT in humans and  Est2 in budding yeast), a template RNA (hTERC in humans and Tlc1 in yeast), and accessory  factors (the Est1 proteins and dyskerin in humans and Est1, Est3, and Sm proteins  in budding yeast).	gene_phenotype
72398	18	334619	5	NULL	NULL	0	NULL	statement 17	Process		occurs along with					statement 14	Process				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_177_s_14	15189140	Telomeres are composed of repetitive sequences that can be maintained  by telomerase, a complex containing a reverse transcriptase (hTERT in humans and  Est2 in budding yeast), a template RNA (hTERC in humans and Tlc1 in yeast), and accessory  factors (the Est1 proteins and dyskerin in humans and Est1, Est3, and Sm proteins  in budding yeast).	gene_phenotype
72399	19	334619	5	NULL	NULL	0	NULL	hTERT	GP		is a type of					reverse transcriptase	GP				NULL	human	0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_177_s_14	15189140	Telomeres are composed of repetitive sequences that can be maintained  by telomerase, a complex containing a reverse transcriptase (hTERT in humans and  Est2 in budding yeast), a template RNA (hTERC in humans and Tlc1 in yeast), and accessory  factors (the Est1 proteins and dyskerin in humans and Est1, Est3, and Sm proteins  in budding yeast).	gene_phenotype
72400	20	334619	5	NULL	NULL	0	NULL	Est2	GP		is a type of					reverse transcriptase	GP				NULL	budding yeast	0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_177_s_14	15189140	Telomeres are composed of repetitive sequences that can be maintained  by telomerase, a complex containing a reverse transcriptase (hTERT in humans and  Est2 in budding yeast), a template RNA (hTERC in humans and Tlc1 in yeast), and accessory  factors (the Est1 proteins and dyskerin in humans and Est1, Est3, and Sm proteins  in budding yeast).	gene_phenotype
72401	21	334619	5	NULL	NULL	0	NULL	hTERC	NucleicAcid		is a type of					template RNA	NucleicAcid				NULL	human	0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_177_s_14	15189140	Telomeres are composed of repetitive sequences that can be maintained  by telomerase, a complex containing a reverse transcriptase (hTERT in humans and  Est2 in budding yeast), a template RNA (hTERC in humans and Tlc1 in yeast), and accessory  factors (the Est1 proteins and dyskerin in humans and Est1, Est3, and Sm proteins  in budding yeast).	gene_phenotype
72402	22	334619	5	NULL	NULL	0	NULL	Tlc1	NucleicAcid		is a type of					template RNA	NucleicAcid				NULL	budding yeast	0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_177_s_14	15189140	Telomeres are composed of repetitive sequences that can be maintained  by telomerase, a complex containing a reverse transcriptase (hTERT in humans and  Est2 in budding yeast), a template RNA (hTERC in humans and Tlc1 in yeast), and accessory  factors (the Est1 proteins and dyskerin in humans and Est1, Est3, and Sm proteins  in budding yeast).	gene_phenotype
72403	23	334619	5	NULL	NULL	0	NULL	Est1 protein	GP		is a type of					accessory factor	GP				NULL	human	0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_177_s_14	15189140	Telomeres are composed of repetitive sequences that can be maintained  by telomerase, a complex containing a reverse transcriptase (hTERT in humans and  Est2 in budding yeast), a template RNA (hTERC in humans and Tlc1 in yeast), and accessory  factors (the Est1 proteins and dyskerin in humans and Est1, Est3, and Sm proteins  in budding yeast).	gene_phenotype
72404	24	334619	5	NULL	NULL	0	NULL	dyskerin	GP		is a type of					accessory factor	GP				NULL	human	0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_177_s_14	15189140	Telomeres are composed of repetitive sequences that can be maintained  by telomerase, a complex containing a reverse transcriptase (hTERT in humans and  Est2 in budding yeast), a template RNA (hTERC in humans and Tlc1 in yeast), and accessory  factors (the Est1 proteins and dyskerin in humans and Est1, Est3, and Sm proteins  in budding yeast).	gene_phenotype
72405	25	334619	5	NULL	NULL	0	NULL	Est1 protein	GP		is a type of					accessory factor	GP				NULL	budding yeast	0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_177_s_14	15189140	Telomeres are composed of repetitive sequences that can be maintained  by telomerase, a complex containing a reverse transcriptase (hTERT in humans and  Est2 in budding yeast), a template RNA (hTERC in humans and Tlc1 in yeast), and accessory  factors (the Est1 proteins and dyskerin in humans and Est1, Est3, and Sm proteins  in budding yeast).	gene_phenotype
72406	26	334619	5	NULL	NULL	0	NULL	Est3 protein	GP		is a type of					accessory factor	GP				NULL	budding yeast	0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_177_s_14	15189140	Telomeres are composed of repetitive sequences that can be maintained  by telomerase, a complex containing a reverse transcriptase (hTERT in humans and  Est2 in budding yeast), a template RNA (hTERC in humans and Tlc1 in yeast), and accessory  factors (the Est1 proteins and dyskerin in humans and Est1, Est3, and Sm proteins  in budding yeast).	gene_phenotype
72407	27	334619	5	NULL	NULL	0	NULL	Sm protein	GP		is a type of					accessory factor	GP				NULL	budding yeast	0	NULL	NULL	NULL	gw70_annurevbiochem_73_0_177_s_14	15189140	Telomeres are composed of repetitive sequences that can be maintained  by telomerase, a complex containing a reverse transcriptase (hTERT in humans and  Est2 in budding yeast), a template RNA (hTERC in humans and Tlc1 in yeast), and accessory  factors (the Est1 proteins and dyskerin in humans and Est1, Est3, and Sm proteins  in budding yeast).	gene_phenotype
72408	1	334620	5	NULL	NULL	0	NULL	yKu80-135i 	GP	mutation of	leads to					telomere	Chromosome	accelerated loss of;; length			NULL	budding yeast strains	0	NULL	NULL	NULL	gw70_nucleicacidsres_33_7_2090_s_205	15824061	Budding yeast strains harboring the  yKu80-135i mutation or  tlc1delta 48 (TLC1 lacking 48 nt Ku binding stem - loop) show accelerated loss of telomere length, which is not attributed to loss of telomerase activity but to reduced kinetics of telomere addition ( ).	gene_phenotype
72409	2	334620	5	NULL	NULL	0	NULL	tlc1delta 48	NucleicAcid	mutation of	leads to					telomere	Chromosome	accelerated loss of;; length			NULL	budding yeast strains	0	NULL	NULL	NULL	gw70_nucleicacidsres_33_7_2090_s_205	15824061	Budding yeast strains harboring the  yKu80-135i mutation or  tlc1delta 48 (TLC1 lacking 48 nt Ku binding stem - loop) show accelerated loss of telomere length, which is not attributed to loss of telomerase activity but to reduced kinetics of telomere addition ( ).	gene_phenotype
72410	3	334620	5	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL	budding yeast strains	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_7_2090_s_205	15824061	Budding yeast strains harboring the  yKu80-135i mutation or  tlc1delta 48 (TLC1 lacking 48 nt Ku binding stem - loop) show accelerated loss of telomere length, which is not attributed to loss of telomerase activity but to reduced kinetics of telomere addition ( ).	gene_phenotype
72411	4	334620	5	NULL	NULL	0	NULL	tlc1delta 48	NucleicAcid		is					TLC1 lacking 48 nt Ku binding stem - loop	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_7_2090_s_205	15824061	Budding yeast strains harboring the  yKu80-135i mutation or  tlc1delta 48 (TLC1 lacking 48 nt Ku binding stem - loop) show accelerated loss of telomere length, which is not attributed to loss of telomerase activity but to reduced kinetics of telomere addition ( ).	gene_phenotype
72412	5	334620	5	NULL	NULL	NULL	NULL	statement 1	Process		is not attributed to					telomere activity	Process	loss of			NULL	budding yeast strains	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_7_2090_s_205	15824061	Budding yeast strains harboring the  yKu80-135i mutation or  tlc1delta 48 (TLC1 lacking 48 nt Ku binding stem - loop) show accelerated loss of telomere length, which is not attributed to loss of telomerase activity but to reduced kinetics of telomere addition ( ).	gene_phenotype
72413	6	334620	5	NULL	NULL	NULL	NULL	statement 1	Process		is attributed to					telomere	Chromosome	reduced kinetics of;;addition of			NULL	budding yeast strains	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_7_2090_s_205	15824061	Budding yeast strains harboring the  yKu80-135i mutation or  tlc1delta 48 (TLC1 lacking 48 nt Ku binding stem - loop) show accelerated loss of telomere length, which is not attributed to loss of telomerase activity but to reduced kinetics of telomere addition ( ).	gene_phenotype
72414	7	334620	5	NULL	NULL	NULL	NULL	statement 2	Process		is not attributed to					telomere activity	Process	loss of			NULL	budding yeast strains	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_7_2090_s_205	15824061	Budding yeast strains harboring the  yKu80-135i mutation or  tlc1delta 48 (TLC1 lacking 48 nt Ku binding stem - loop) show accelerated loss of telomere length, which is not attributed to loss of telomerase activity but to reduced kinetics of telomere addition ( ).	gene_phenotype
72415	8	334620	5	NULL	NULL	NULL	NULL	statement 2	Process		is attributed to					telomere	Chromosome	reduced kinetics of;;addition of			NULL	budding yeast strains	NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_7_2090_s_205	15824061	Budding yeast strains harboring the  yKu80-135i mutation or  tlc1delta 48 (TLC1 lacking 48 nt Ku binding stem - loop) show accelerated loss of telomere length, which is not attributed to loss of telomerase activity but to reduced kinetics of telomere addition ( ).	gene_phenotype
72416	1	334623	5	NULL	NULL	0	NULL	telomere	Chromosome	progressive shortening of	is accompanied by					cell viability	Process	gradual loss of			NULL	delta tlc1	0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8729_s_30	14612413	Yeast cells defective in the telomerase pathway, as the  Saccharomyces cerevisiae mutants delta tlc1 and  deltaest1- 4 or the  Kluyveromyces lactis telomerase mutant delta ter1 show a phenotype very similar to that seen in mammalian cells: progressive telomere shortening accompanied by gradual loss of cell viability through a senescence-like mechanism ( ,  ,  ,  ).	gene_phenotype
72417	2	334623	5	NULL	NULL	0	NULL	statement 1	Process		occurs through					senescence-like mechanism	Process				NULL	delta tlc1	0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8729_s_30	14612413	Yeast cells defective in the telomerase pathway, as the  Saccharomyces cerevisiae mutants delta tlc1 and  deltaest1- 4 or the  Kluyveromyces lactis telomerase mutant delta ter1 show a phenotype very similar to that seen in mammalian cells: progressive telomere shortening accompanied by gradual loss of cell viability through a senescence-like mechanism ( ,  ,  ,  ).	gene_phenotype
72418	3	334623	5	NULL	NULL	NULL	NULL	telomere	Chromosome	progressive shortening of	is accompanied by					cell viability	Process	gradual loss of			NULL	deltaest1- 4	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8729_s_30	14612413	Yeast cells defective in the telomerase pathway, as the  Saccharomyces cerevisiae mutants delta tlc1 and  deltaest1- 4 or the  Kluyveromyces lactis telomerase mutant delta ter1 show a phenotype very similar to that seen in mammalian cells: progressive telomere shortening accompanied by gradual loss of cell viability through a senescence-like mechanism ( ,  ,  ,  ).	gene_phenotype
72419	4	334623	5	NULL	NULL	0	NULL	statement 3	Process		occurs through					senescence-like mechanism	Process				NULL	deltaest1- 4	0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8729_s_30	14612413	Yeast cells defective in the telomerase pathway, as the  Saccharomyces cerevisiae mutants delta tlc1 and  deltaest1- 4 or the  Kluyveromyces lactis telomerase mutant delta ter1 show a phenotype very similar to that seen in mammalian cells: progressive telomere shortening accompanied by gradual loss of cell viability through a senescence-like mechanism ( ,  ,  ,  ).	gene_phenotype
72420	5	334623	5	NULL	NULL	NULL	NULL	telomere	Chromosome	progressive shortening of	is accompanied by					cell viability	Process	gradual loss of			NULL	delta ter1	NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8729_s_30	14612413	Yeast cells defective in the telomerase pathway, as the  Saccharomyces cerevisiae mutants delta tlc1 and  deltaest1- 4 or the  Kluyveromyces lactis telomerase mutant delta ter1 show a phenotype very similar to that seen in mammalian cells: progressive telomere shortening accompanied by gradual loss of cell viability through a senescence-like mechanism ( ,  ,  ,  ).	gene_phenotype
72421	6	334623	5	NULL	NULL	0	NULL	statement 5	Process		occurs through					senescence-like mechanism	Process				NULL	delta ter1	0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8729_s_30	14612413	Yeast cells defective in the telomerase pathway, as the  Saccharomyces cerevisiae mutants delta tlc1 and  deltaest1- 4 or the  Kluyveromyces lactis telomerase mutant delta ter1 show a phenotype very similar to that seen in mammalian cells: progressive telomere shortening accompanied by gradual loss of cell viability through a senescence-like mechanism ( ,  ,  ,  ).	gene_phenotype
72422	7	334623	5	NULL	NULL	0	NULL	delta tlc1	Organism		is a mutant of					Saccharomyces cerevisiae	Organism				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8729_s_30	14612413	Yeast cells defective in the telomerase pathway, as the  Saccharomyces cerevisiae mutants delta tlc1 and  deltaest1- 4 or the  Kluyveromyces lactis telomerase mutant delta ter1 show a phenotype very similar to that seen in mammalian cells: progressive telomere shortening accompanied by gradual loss of cell viability through a senescence-like mechanism ( ,  ,  ,  ).	gene_phenotype
72423	8	334623	5	NULL	NULL	0	NULL	statement 7	Organism		is defective in					telomerase pathway	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8729_s_30	14612413	Yeast cells defective in the telomerase pathway, as the  Saccharomyces cerevisiae mutants delta tlc1 and  deltaest1- 4 or the  Kluyveromyces lactis telomerase mutant delta ter1 show a phenotype very similar to that seen in mammalian cells: progressive telomere shortening accompanied by gradual loss of cell viability through a senescence-like mechanism ( ,  ,  ,  ).	gene_phenotype
72424	9	334623	5	NULL	NULL	0	NULL	deltaest1- 4	Organism		is a mutant of					Saccharomyces cerevisiae	Organism				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8729_s_30	14612413	Yeast cells defective in the telomerase pathway, as the  Saccharomyces cerevisiae mutants delta tlc1 and  deltaest1- 4 or the  Kluyveromyces lactis telomerase mutant delta ter1 show a phenotype very similar to that seen in mammalian cells: progressive telomere shortening accompanied by gradual loss of cell viability through a senescence-like mechanism ( ,  ,  ,  ).	gene_phenotype
72425	10	334623	5	NULL	NULL	0	NULL	statement 9	Process		is defective in					telomerase pathway	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8729_s_30	14612413	Yeast cells defective in the telomerase pathway, as the  Saccharomyces cerevisiae mutants delta tlc1 and  deltaest1- 4 or the  Kluyveromyces lactis telomerase mutant delta ter1 show a phenotype very similar to that seen in mammalian cells: progressive telomere shortening accompanied by gradual loss of cell viability through a senescence-like mechanism ( ,  ,  ,  ).	gene_phenotype
72426	11	334623	5	NULL	NULL	0	NULL	delta ter1	Organism		is a mutant of					Kluyveromyces lactis	Organism				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8729_s_30	14612413	Yeast cells defective in the telomerase pathway, as the  Saccharomyces cerevisiae mutants delta tlc1 and  deltaest1- 4 or the  Kluyveromyces lactis telomerase mutant delta ter1 show a phenotype very similar to that seen in mammalian cells: progressive telomere shortening accompanied by gradual loss of cell viability through a senescence-like mechanism ( ,  ,  ,  ).	gene_phenotype
72427	12	334623	5	NULL	NULL	0	NULL	statement 11	Organism		is defective in					telomerase pathway	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8729_s_30	14612413	Yeast cells defective in the telomerase pathway, as the  Saccharomyces cerevisiae mutants delta tlc1 and  deltaest1- 4 or the  Kluyveromyces lactis telomerase mutant delta ter1 show a phenotype very similar to that seen in mammalian cells: progressive telomere shortening accompanied by gradual loss of cell viability through a senescence-like mechanism ( ,  ,  ,  ).	gene_phenotype
72428	1	334625	5	NULL	NULL	0	NULL	Gnop1	GP		is an ortholog of					PinX1	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_50_51745_s_131	15381700	In the budding yeast, the PinX1 orthologue Gnop1 appears to inhibit telomerase biogenesis by sequestering the uncomplexed TERT protein (Est2p) and preventing its association with the telomerase template RNA (TLC1) ( ), consistent with the localization of this protein to the nucleolus ( ) where telomerase assembly is believed to occur.	gene_phenotype
72429	2	334625	5	NULL	NULL	0	NULL	Gnop1	GP		inhibits		appear to			telomerase	GP	biogenesis of			NULL	budding yeast	0	NULL	NULL	NULL	gw70_jbiolchem_279_50_51745_s_131	15381700	In the budding yeast, the PinX1 orthologue Gnop1 appears to inhibit telomerase biogenesis by sequestering the uncomplexed TERT protein (Est2p) and preventing its association with the telomerase template RNA (TLC1) ( ), consistent with the localization of this protein to the nucleolus ( ) where telomerase assembly is believed to occur.	gene_phenotype
72430	3	334625	5	NULL	NULL	0	NULL	Gnop1	GP		sequester					TERT protein	GP	uncomplexed			NULL	budding yeast	0	NULL	NULL	NULL	gw70_jbiolchem_279_50_51745_s_131	15381700	In the budding yeast, the PinX1 orthologue Gnop1 appears to inhibit telomerase biogenesis by sequestering the uncomplexed TERT protein (Est2p) and preventing its association with the telomerase template RNA (TLC1) ( ), consistent with the localization of this protein to the nucleolus ( ) where telomerase assembly is believed to occur.	gene_phenotype
72434	4	334625	5	NULL	NULL	0	NULL	TERT protein	GP		associates with					TLC1	NucleicAcid				NULL	budding yeast	0	NULL	NULL	NULL	gw70_jbiolchem_279_50_51745_s_131	15381700	In the budding yeast, the PinX1 orthologue Gnop1 appears to inhibit telomerase biogenesis by sequestering the uncomplexed TERT protein (Est2p) and preventing its association with the telomerase template RNA (TLC1) ( ), consistent with the localization of this protein to the nucleolus ( ) where telomerase assembly is believed to occur.	gene_phenotype
72435	5	334625	5	NULL	NULL	0	NULL	statement 3	Process		prevent					statement 4	Process				NULL	budding yeast	0	NULL	NULL	NULL	gw70_jbiolchem_279_50_51745_s_131	15381700	In the budding yeast, the PinX1 orthologue Gnop1 appears to inhibit telomerase biogenesis by sequestering the uncomplexed TERT protein (Est2p) and preventing its association with the telomerase template RNA (TLC1) ( ), consistent with the localization of this protein to the nucleolus ( ) where telomerase assembly is believed to occur.	gene_phenotype
72436	6	334625	5	NULL	NULL	0	NULL	statement 5	Process		leads to					statement 2	Process				NULL	budding yeast	0	NULL	NULL	NULL	gw70_jbiolchem_279_50_51745_s_131	15381700	In the budding yeast, the PinX1 orthologue Gnop1 appears to inhibit telomerase biogenesis by sequestering the uncomplexed TERT protein (Est2p) and preventing its association with the telomerase template RNA (TLC1) ( ), consistent with the localization of this protein to the nucleolus ( ) where telomerase assembly is believed to occur.	gene_phenotype
72437	7	334625	5	NULL	NULL	0	NULL	Gnop1	GP		is localized to					nucleolus	CellComponent				NULL	budding yeast	0	NULL	NULL	NULL	gw70_jbiolchem_279_50_51745_s_131	15381700	In the budding yeast, the PinX1 orthologue Gnop1 appears to inhibit telomerase biogenesis by sequestering the uncomplexed TERT protein (Est2p) and preventing its association with the telomerase template RNA (TLC1) ( ), consistent with the localization of this protein to the nucleolus ( ) where telomerase assembly is believed to occur.	gene_phenotype
72438	8	334625	5	NULL	NULL	0	NULL	telomerase	GP	assembly of	occurs in		possibly			nucleolus	CellComponent				NULL	budding yeast	0	NULL	NULL	NULL	gw70_jbiolchem_279_50_51745_s_131	15381700	In the budding yeast, the PinX1 orthologue Gnop1 appears to inhibit telomerase biogenesis by sequestering the uncomplexed TERT protein (Est2p) and preventing its association with the telomerase template RNA (TLC1) ( ), consistent with the localization of this protein to the nucleolus ( ) where telomerase assembly is believed to occur.	gene_phenotype
72439	9	334625	5	NULL	NULL	0	NULL	Est2p	GP		is a synonym of					TERT protein	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_50_51745_s_131	15381700	In the budding yeast, the PinX1 orthologue Gnop1 appears to inhibit telomerase biogenesis by sequestering the uncomplexed TERT protein (Est2p) and preventing its association with the telomerase template RNA (TLC1) ( ), consistent with the localization of this protein to the nucleolus ( ) where telomerase assembly is believed to occur.	gene_phenotype
72440	10	334625	5	NULL	NULL	0	NULL	TLC1	NucleicAcid		is a type of					telomere template	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_50_51745_s_131	15381700	In the budding yeast, the PinX1 orthologue Gnop1 appears to inhibit telomerase biogenesis by sequestering the uncomplexed TERT protein (Est2p) and preventing its association with the telomerase template RNA (TLC1) ( ), consistent with the localization of this protein to the nucleolus ( ) where telomerase assembly is believed to occur.	gene_phenotype
72441	1	334626	5	NULL	NULL	0	NULL	TLC1 RNA	NucleicAcid		is associated with					TERT	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_6_3882_s_142	12458198	Mutations in the CP, QFP, and T Motifs Caused a Reduction in the Amount of TERT Protein  and TERT-associated TLC1 RNA-- To determine the basis for the activity loss manifested by the SCR mutants, we estimated  the levels of TERT protein in wild type and mutant strains using antibodies directed against the protein A tag.	gene_phenotype
72442	2	334626	5	NULL	NULL	NULL	NULL	CP motif	AminoAcid	mutation of	reduce					TERT protein	GP	amount of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_6_3882_s_142	12458198	Mutations in the CP, QFP, and T Motifs Caused a Reduction in the Amount of TERT Protein  and TERT-associated TLC1 RNA-- To determine the basis for the activity loss manifested by the SCR mutants, we estimated  the levels of TERT protein in wild type and mutant strains using antibodies directed against the protein A tag.	gene_phenotype
72443	3	334626	5	NULL	NULL	NULL	NULL	CP motif	AminoAcid	mutation of	reduce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_6_3882_s_142	12458198	Mutations in the CP, QFP, and T Motifs Caused a Reduction in the Amount of TERT Protein  and TERT-associated TLC1 RNA-- To determine the basis for the activity loss manifested by the SCR mutants, we estimated  the levels of TERT protein in wild type and mutant strains using antibodies directed against the protein A tag.	gene_phenotype
72444	4	334626	5	NULL	NULL	NULL	NULL	QFP motif	AminoAcid	mutation of	reduce					TERT protein	GP	amount of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_6_3882_s_142	12458198	Mutations in the CP, QFP, and T Motifs Caused a Reduction in the Amount of TERT Protein  and TERT-associated TLC1 RNA-- To determine the basis for the activity loss manifested by the SCR mutants, we estimated  the levels of TERT protein in wild type and mutant strains using antibodies directed against the protein A tag.	gene_phenotype
72445	5	334626	5	NULL	NULL	NULL	NULL	QFP motif	AminoAcid	mutation of	reduce					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_6_3882_s_142	12458198	Mutations in the CP, QFP, and T Motifs Caused a Reduction in the Amount of TERT Protein  and TERT-associated TLC1 RNA-- To determine the basis for the activity loss manifested by the SCR mutants, we estimated  the levels of TERT protein in wild type and mutant strains using antibodies directed against the protein A tag.	gene_phenotype
72446	6	334626	5	NULL	NULL	0	NULL	T Motif	AminoAcid	mutation of	reduce					TERT protein	GP	amount of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_6_3882_s_142	12458198	Mutations in the CP, QFP, and T Motifs Caused a Reduction in the Amount of TERT Protein  and TERT-associated TLC1 RNA-- To determine the basis for the activity loss manifested by the SCR mutants, we estimated  the levels of TERT protein in wild type and mutant strains using antibodies directed against the protein A tag.	gene_phenotype
72447	7	334626	5	NULL	NULL	0	NULL	T Motif	AminoAcid	mutation of	reduce					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_6_3882_s_142	12458198	Mutations in the CP, QFP, and T Motifs Caused a Reduction in the Amount of TERT Protein  and TERT-associated TLC1 RNA-- To determine the basis for the activity loss manifested by the SCR mutants, we estimated  the levels of TERT protein in wild type and mutant strains using antibodies directed against the protein A tag.	gene_phenotype
72448	1	334627	5	NULL	NULL	NULL	NULL	CP motif	AminoAcid	mutation of	affects					RNP	GP	assembly of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_6_3882_s_176	12458198	Overexpression of the Mutant Proteins Does Not Result in Telomere Shortening-- The concomitant reduction in the level of telomerase activity, TERT protein, and  TERT-associated TLC1 RNA suggests that mutations in the CP, QFP, and T motifs affected RNP assembly rather than the  in vivo and  in vitro activity of telomerase.	gene_phenotype
72449	2	334627	5	NULL	NULL	0	NULL	QFP motif	AminoAcid	mutation of	affects					RNP	GP	assembly of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_6_3882_s_176	12458198	Overexpression of the Mutant Proteins Does Not Result in Telomere Shortening-- The concomitant reduction in the level of telomerase activity, TERT protein, and  TERT-associated TLC1 RNA suggests that mutations in the CP, QFP, and T motifs affected RNP assembly rather than the  in vivo and  in vitro activity of telomerase.	gene_phenotype
72450	3	334627	5	NULL	NULL	0	NULL	T motif	AminoAcid	mutation of	affects					RNP	GP	assembly of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_6_3882_s_176	12458198	Overexpression of the Mutant Proteins Does Not Result in Telomere Shortening-- The concomitant reduction in the level of telomerase activity, TERT protein, and  TERT-associated TLC1 RNA suggests that mutations in the CP, QFP, and T motifs affected RNP assembly rather than the  in vivo and  in vitro activity of telomerase.	gene_phenotype
72451	4	334627	5	NULL	NULL	0	NULL	CP motif	AminoAcid	mutation of	does not affect					telomere activity	Process				NULL	in vitro	0	NULL	NULL	NULL	gw70_jbiolchem_278_6_3882_s_176	12458198	Overexpression of the Mutant Proteins Does Not Result in Telomere Shortening-- The concomitant reduction in the level of telomerase activity, TERT protein, and  TERT-associated TLC1 RNA suggests that mutations in the CP, QFP, and T motifs affected RNP assembly rather than the  in vivo and  in vitro activity of telomerase.	gene_phenotype
72452	5	334627	5	NULL	NULL	0	NULL	CP motif	AminoAcid	mutation of	does not affect					telomere activity	Process				NULL	in vivo	0	NULL	NULL	NULL	gw70_jbiolchem_278_6_3882_s_176	12458198	Overexpression of the Mutant Proteins Does Not Result in Telomere Shortening-- The concomitant reduction in the level of telomerase activity, TERT protein, and  TERT-associated TLC1 RNA suggests that mutations in the CP, QFP, and T motifs affected RNP assembly rather than the  in vivo and  in vitro activity of telomerase.	gene_phenotype
72453	6	334627	5	NULL	NULL	0	NULL	QFP motif	AminoAcid	mutation of	does not affect					telomere activity	Process				NULL	in vitro	0	NULL	NULL	NULL	gw70_jbiolchem_278_6_3882_s_176	12458198	Overexpression of the Mutant Proteins Does Not Result in Telomere Shortening-- The concomitant reduction in the level of telomerase activity, TERT protein, and  TERT-associated TLC1 RNA suggests that mutations in the CP, QFP, and T motifs affected RNP assembly rather than the  in vivo and  in vitro activity of telomerase.	gene_phenotype
72454	7	334627	5	NULL	NULL	0	NULL	QFP motif	AminoAcid	mutation of	does not affect					telomere activity	Process				NULL	in vivo	0	NULL	NULL	NULL	gw70_jbiolchem_278_6_3882_s_176	12458198	Overexpression of the Mutant Proteins Does Not Result in Telomere Shortening-- The concomitant reduction in the level of telomerase activity, TERT protein, and  TERT-associated TLC1 RNA suggests that mutations in the CP, QFP, and T motifs affected RNP assembly rather than the  in vivo and  in vitro activity of telomerase.	gene_phenotype
72455	8	334627	5	NULL	NULL	0	NULL	T Motif	AminoAcid	mutation of	does not affect					telomere activity	Process				NULL	in vitro	0	NULL	NULL	NULL	gw70_jbiolchem_278_6_3882_s_176	12458198	Overexpression of the Mutant Proteins Does Not Result in Telomere Shortening-- The concomitant reduction in the level of telomerase activity, TERT protein, and  TERT-associated TLC1 RNA suggests that mutations in the CP, QFP, and T motifs affected RNP assembly rather than the  in vivo and  in vitro activity of telomerase.	gene_phenotype
72456	9	334627	5	NULL	NULL	0	NULL	T Motif	AminoAcid	mutation of	does not affect					telomere activity	Process				NULL	in vivo	0	NULL	NULL	NULL	gw70_jbiolchem_278_6_3882_s_176	12458198	Overexpression of the Mutant Proteins Does Not Result in Telomere Shortening-- The concomitant reduction in the level of telomerase activity, TERT protein, and  TERT-associated TLC1 RNA suggests that mutations in the CP, QFP, and T motifs affected RNP assembly rather than the  in vivo and  in vitro activity of telomerase.	gene_phenotype
72457	1	334629	5	NULL	NULL	0	NULL	telomerase	GP		consists of			catalytic core		TLC1	NucleicAcid	Saccharomyces cerevisiae			NULL		0	NULL	NULL	NULL	gw70_pnas_102_28_9778_s_9	15994230	The catalytic core of telomerase consists minimally of two components: an RNA in which the template is embedded (named TLC1 in the budding yeast  Saccharomyces cerevisiae), and a reverse transcriptase (RT)-like protein that mediates catalysis (named TERT in general and Est2p in yeast) (  -  ).	gene_phenotype
72458	2	334629	5	NULL	NULL	0	NULL	TLC1	NucleicAcid	Saccharomyces cerevisiae	is a type of					RNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_pnas_102_28_9778_s_9	15994230	The catalytic core of telomerase consists minimally of two components: an RNA in which the template is embedded (named TLC1 in the budding yeast  Saccharomyces cerevisiae), and a reverse transcriptase (RT)-like protein that mediates catalysis (named TERT in general and Est2p in yeast) (  -  ).	gene_phenotype
72459	3	334629	5	NULL	NULL	0	NULL	telomerase	GP		consists of			catalytic core		TERT	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_102_28_9778_s_9	15994230	The catalytic core of telomerase consists minimally of two components: an RNA in which the template is embedded (named TLC1 in the budding yeast  Saccharomyces cerevisiae), and a reverse transcriptase (RT)-like protein that mediates catalysis (named TERT in general and Est2p in yeast) (  -  ).	gene_phenotype
72460	4	334629	5	NULL	NULL	0	NULL	telomerase	GP		consists of			catalytic core		Est2p	GP	yeast			NULL		0	NULL	NULL	NULL	gw70_pnas_102_28_9778_s_9	15994230	The catalytic core of telomerase consists minimally of two components: an RNA in which the template is embedded (named TLC1 in the budding yeast  Saccharomyces cerevisiae), and a reverse transcriptase (RT)-like protein that mediates catalysis (named TERT in general and Est2p in yeast) (  -  ).	gene_phenotype
72461	5	334629	5	NULL	NULL	0	NULL	TERT	GP		is a type of					reverse transcriptase like protein	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_102_28_9778_s_9	15994230	The catalytic core of telomerase consists minimally of two components: an RNA in which the template is embedded (named TLC1 in the budding yeast  Saccharomyces cerevisiae), and a reverse transcriptase (RT)-like protein that mediates catalysis (named TERT in general and Est2p in yeast) (  -  ).	gene_phenotype
72462	6	334629	5	NULL	NULL	0	NULL	Est2p	GP	yeast	is a type of					reverse transcriptase like protein	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_102_28_9778_s_9	15994230	The catalytic core of telomerase consists minimally of two components: an RNA in which the template is embedded (named TLC1 in the budding yeast  Saccharomyces cerevisiae), and a reverse transcriptase (RT)-like protein that mediates catalysis (named TERT in general and Est2p in yeast) (  -  ).	gene_phenotype
72463	7	334629	5	NULL	NULL	0	NULL	statement 5	Process		mediates					catalysis	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_102_28_9778_s_9	15994230	The catalytic core of telomerase consists minimally of two components: an RNA in which the template is embedded (named TLC1 in the budding yeast  Saccharomyces cerevisiae), and a reverse transcriptase (RT)-like protein that mediates catalysis (named TERT in general and Est2p in yeast) (  -  ).	gene_phenotype
72464	8	334629	5	NULL	NULL	0	NULL	statement 6	Process		mediates					catalysis	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_102_28_9778_s_9	15994230	The catalytic core of telomerase consists minimally of two components: an RNA in which the template is embedded (named TLC1 in the budding yeast  Saccharomyces cerevisiae), and a reverse transcriptase (RT)-like protein that mediates catalysis (named TERT in general and Est2p in yeast) (  -  ).	gene_phenotype
72465	1	334630	5	NULL	NULL	0	NULL	TLC1	NucleicAcid	deletion of;;either side of;;predicted;;S. cerevisiae	decrease		modestly		 helix 4	telomere	Chromosome	length of			NULL		0	NULL	NULL	NULL	gw70_pnas_101_41_14713_s_128	15371596	Deletion of either side of predicted helix 4 in  S. cerevisiae TLC1 (mutants 12, 13, and 170) or changing the sequences surrounding helix 4 (mutants 14, 15, and 16) only modestly decreased telomere length or cell growth ( Fig. 2 and Tables 1 and 2).	gene_phenotype
72466	2	334630	5	NULL	NULL	0	NULL	TLC1	NucleicAcid	deletion of;;either side of;;predicted;;S. cerevisiae	decrease		modestly		helix 4	cell growth	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_101_41_14713_s_128	15371596	Deletion of either side of predicted helix 4 in  S. cerevisiae TLC1 (mutants 12, 13, and 170) or changing the sequences surrounding helix 4 (mutants 14, 15, and 16) only modestly decreased telomere length or cell growth ( Fig. 2 and Tables 1 and 2).	gene_phenotype
72467	3	334630	5	NULL	NULL	0	NULL	TLC1	NucleicAcid	changing sequence surrounding	decrease		modestly		helix 4	telomere	Chromosome	length of			NULL		0	NULL	NULL	NULL	gw70_pnas_101_41_14713_s_128	15371596	Deletion of either side of predicted helix 4 in  S. cerevisiae TLC1 (mutants 12, 13, and 170) or changing the sequences surrounding helix 4 (mutants 14, 15, and 16) only modestly decreased telomere length or cell growth ( Fig. 2 and Tables 1 and 2).	gene_phenotype
72468	4	334630	5	NULL	NULL	0	NULL	TLC1	NucleicAcid	changing sequence surrounding	decrease		modestly		helix 4	cell growth	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_101_41_14713_s_128	15371596	Deletion of either side of predicted helix 4 in  S. cerevisiae TLC1 (mutants 12, 13, and 170) or changing the sequences surrounding helix 4 (mutants 14, 15, and 16) only modestly decreased telomere length or cell growth ( Fig. 2 and Tables 1 and 2).	gene_phenotype
72469	5	334630	5	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_101_41_14713_s_128	15371596	Deletion of either side of predicted helix 4 in  S. cerevisiae TLC1 (mutants 12, 13, and 170) or changing the sequences surrounding helix 4 (mutants 14, 15, and 16) only modestly decreased telomere length or cell growth ( Fig. 2 and Tables 1 and 2).	gene_phenotype
72470	6	334630	5	NULL	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_101_41_14713_s_128	15371596	Deletion of either side of predicted helix 4 in  S. cerevisiae TLC1 (mutants 12, 13, and 170) or changing the sequences surrounding helix 4 (mutants 14, 15, and 16) only modestly decreased telomere length or cell growth ( Fig. 2 and Tables 1 and 2).	gene_phenotype
72471	1	334632	5	NULL	NULL	0	NULL	Est1p	GP		activates		nonspecific			RNA	NucleicAcid	binding of			NULL	in vitro	0	NULL	NULL	NULL	gw60_genesdev_12_8_1073_s_147	9553037	Est1p also exhibits a nonspecific RNA binding activity in vitro, with no enhanced binding to the  TLC1 telomerase RNA (Virta-Pearlman et al. 1996  ), although this lack of specificity could be the result of incorrect folding of the 1.3-kb yeast telomerase RNA or the lack of another protein binding partner.	gene_phenotype
72472	2	334632	5	NULL	NULL	0	NULL	Est1p	GP		does not bind					TLC1	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_8_1073_s_147	9553037	Est1p also exhibits a nonspecific RNA binding activity in vitro, with no enhanced binding to the  TLC1 telomerase RNA (Virta-Pearlman et al. 1996  ), although this lack of specificity could be the result of incorrect folding of the 1.3-kb yeast telomerase RNA or the lack of another protein binding partner.	gene_phenotype
72473	3	334632	5	NULL	NULL	0	NULL	TLC1	NucleicAcid		is a type of					telomerase RNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_8_1073_s_147	9553037	Est1p also exhibits a nonspecific RNA binding activity in vitro, with no enhanced binding to the  TLC1 telomerase RNA (Virta-Pearlman et al. 1996  ), although this lack of specificity could be the result of incorrect folding of the 1.3-kb yeast telomerase RNA or the lack of another protein binding partner.	gene_phenotype
72474	4	334632	5	NULL	NULL	0	NULL	telomerase RNA	NucleicAcid	incorrect folding of;;yeast	leads to		may			statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_8_1073_s_147	9553037	Est1p also exhibits a nonspecific RNA binding activity in vitro, with no enhanced binding to the  TLC1 telomerase RNA (Virta-Pearlman et al. 1996  ), although this lack of specificity could be the result of incorrect folding of the 1.3-kb yeast telomerase RNA or the lack of another protein binding partner.	gene_phenotype
72475	5	334632	5	NULL	NULL	0	NULL	protein binding partner	GP	lack of	leads to		may			statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_8_1073_s_147	9553037	Est1p also exhibits a nonspecific RNA binding activity in vitro, with no enhanced binding to the  TLC1 telomerase RNA (Virta-Pearlman et al. 1996  ), although this lack of specificity could be the result of incorrect folding of the 1.3-kb yeast telomerase RNA or the lack of another protein binding partner.	gene_phenotype
72476	1	334633	5	NULL	NULL	0	NULL	TLC1 RNA	NucleicAcid		serve as					template	NucleicAcid				NULL	at the ends of yeast chromosomes	0	NULL	NULL	NULL	gw60_genetics_160_1_49_s_149	11805044	TLC1 RNA serves as template for DNA synthesis at the ends of yeast chromosomes during S phase and may have additional functions in telomere silencing and length maintenance ( P RESCOTT and BLACKBURN 1997   ;   S INGER et al. 1998   ;	gene_phenotype
72477	2	334633	5	NULL	NULL	0	NULL	statement 1	Process		is required for					DNA	NucleicAcid	synthesis of			NULL	at the ends of yeast chromosomes	0	NULL	NULL	NULL	gw60_genetics_160_1_49_s_149	11805044	TLC1 RNA serves as template for DNA synthesis at the ends of yeast chromosomes during S phase and may have additional functions in telomere silencing and length maintenance ( P RESCOTT and BLACKBURN 1997   ;   S INGER et al. 1998   ;	gene_phenotype
72478	3	334633	5	NULL	NULL	NULL	NULL	statement 2	Process		occurs during					S phase	Time				NULL	at the ends of yeast chromosomes	NULL	NULL	NULL	NULL	gw60_genetics_160_1_49_s_149	11805044	TLC1 RNA serves as template for DNA synthesis at the ends of yeast chromosomes during S phase and may have additional functions in telomere silencing and length maintenance ( P RESCOTT and BLACKBURN 1997   ;   S INGER et al. 1998   ;	gene_phenotype
72479	4	334633	5	NULL	NULL	0	NULL	statement 2	Process		silence		may			telomere	Chromosome				NULL		0	NULL	NULL	NULL	gw60_genetics_160_1_49_s_149	11805044	TLC1 RNA serves as template for DNA synthesis at the ends of yeast chromosomes during S phase and may have additional functions in telomere silencing and length maintenance ( P RESCOTT and BLACKBURN 1997   ;   S INGER et al. 1998   ;	gene_phenotype
72480	5	334633	5	NULL	NULL	0	NULL	statement 2	Process		maintains		may			telomere	Chromosome	length of			NULL		0	NULL	NULL	NULL	gw60_genetics_160_1_49_s_149	11805044	TLC1 RNA serves as template for DNA synthesis at the ends of yeast chromosomes during S phase and may have additional functions in telomere silencing and length maintenance ( P RESCOTT and BLACKBURN 1997   ;   S INGER et al. 1998   ;	gene_phenotype
72481	1	334637	5	NULL	NULL	0	NULL	tlc1-48 allele	NucleicAcid		impairs					TLC1 activity	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_162_3_1101_s_247	12454059	This epistasis behavior is reminiscent of that of a mutation in another subunit in telomerase: the  tlc1-48 allele impairs an activity of  TLC1 that has been proposed to interact, either directly or indirectly, with the Ku heterodimer to facilitate telomere length maintenance ( P ETERSON et al. 2001   ).	gene_phenotype
72482	2	334637	5	NULL	NULL	0	NULL	TLC1	NucleicAcid		interacts with					Ku heterodimer	GP				NULL		0	NULL	NULL	NULL	gw60_genetics_162_3_1101_s_247	12454059	This epistasis behavior is reminiscent of that of a mutation in another subunit in telomerase: the  tlc1-48 allele impairs an activity of  TLC1 that has been proposed to interact, either directly or indirectly, with the Ku heterodimer to facilitate telomere length maintenance ( P ETERSON et al. 2001   ).	gene_phenotype
72483	3	334637	5	NULL	NULL	0	NULL	statement 2	Process		maintains					telomere	Chromosome	length of			NULL		0	NULL	NULL	NULL	gw60_genetics_162_3_1101_s_247	12454059	This epistasis behavior is reminiscent of that of a mutation in another subunit in telomerase: the  tlc1-48 allele impairs an activity of  TLC1 that has been proposed to interact, either directly or indirectly, with the Ku heterodimer to facilitate telomere length maintenance ( P ETERSON et al. 2001   ).	gene_phenotype
72484	1	334641	5	NULL	NULL	0	NULL	TLC1	NucleicAcid	mutant	causes					lethal phenotype	PhysicalPhenomenon	delayed			NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw60_nucleicacidsres_28_14_2690_s_17	10908324	In the budding yeast  Saccharomyces cerevisiae mutations in the genes coding for the RNA or the protein subunits of telomerase ( TLC1 and  EST1-3, respectively) cause a delayed lethal phenotype after about 75 generations, which is accompanied by progressive telomere shortening ( 8 -  10).	gene_phenotype
72485	2	334641	5	NULL	NULL	0	NULL	statement 1	Process		is accompanied by					telomere	Chromosome	progressive shortening of			NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw60_nucleicacidsres_28_14_2690_s_17	10908324	In the budding yeast  Saccharomyces cerevisiae mutations in the genes coding for the RNA or the protein subunits of telomerase ( TLC1 and  EST1-3, respectively) cause a delayed lethal phenotype after about 75 generations, which is accompanied by progressive telomere shortening ( 8 -  10).	gene_phenotype
72486	3	334641	5	NULL	NULL	0	NULL	EST1	GP	mutant	causes					lethal phenotype	PhysicalPhenomenon	delayed			NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw60_nucleicacidsres_28_14_2690_s_17	10908324	In the budding yeast  Saccharomyces cerevisiae mutations in the genes coding for the RNA or the protein subunits of telomerase ( TLC1 and  EST1-3, respectively) cause a delayed lethal phenotype after about 75 generations, which is accompanied by progressive telomere shortening ( 8 -  10).	gene_phenotype
72487	4	334641	5	NULL	NULL	0	NULL	statement 3	Process		is accompanied by					telomere	Chromosome	progressive shortening of			NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw60_nucleicacidsres_28_14_2690_s_17	10908324	In the budding yeast  Saccharomyces cerevisiae mutations in the genes coding for the RNA or the protein subunits of telomerase ( TLC1 and  EST1-3, respectively) cause a delayed lethal phenotype after about 75 generations, which is accompanied by progressive telomere shortening ( 8 -  10).	gene_phenotype
72488	5	334641	5	NULL	NULL	NULL	NULL	EST2	GP	mutant	causes					lethal phenotype	PhysicalPhenomenon	delayed			NULL	Saccharomyces cerevisiae	NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_14_2690_s_17	10908324	In the budding yeast  Saccharomyces cerevisiae mutations in the genes coding for the RNA or the protein subunits of telomerase ( TLC1 and  EST1-3, respectively) cause a delayed lethal phenotype after about 75 generations, which is accompanied by progressive telomere shortening ( 8 -  10).	gene_phenotype
72489	6	334641	5	NULL	NULL	0	NULL	statement 5	Process		is accompanied by					telomere	Chromosome	progressive shortening of			NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw60_nucleicacidsres_28_14_2690_s_17	10908324	In the budding yeast  Saccharomyces cerevisiae mutations in the genes coding for the RNA or the protein subunits of telomerase ( TLC1 and  EST1-3, respectively) cause a delayed lethal phenotype after about 75 generations, which is accompanied by progressive telomere shortening ( 8 -  10).	gene_phenotype
72490	7	334641	5	NULL	NULL	0	NULL	EST3	GP	mutant	causes					lethal phenotype	PhysicalPhenomenon	delayed			NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw60_nucleicacidsres_28_14_2690_s_17	10908324	In the budding yeast  Saccharomyces cerevisiae mutations in the genes coding for the RNA or the protein subunits of telomerase ( TLC1 and  EST1-3, respectively) cause a delayed lethal phenotype after about 75 generations, which is accompanied by progressive telomere shortening ( 8 -  10).	gene_phenotype
72491	8	334641	5	NULL	NULL	0	NULL	statement 7	Process		is accompanied by					telomere	Chromosome	progressive shortening of			NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	gw60_nucleicacidsres_28_14_2690_s_17	10908324	In the budding yeast  Saccharomyces cerevisiae mutations in the genes coding for the RNA or the protein subunits of telomerase ( TLC1 and  EST1-3, respectively) cause a delayed lethal phenotype after about 75 generations, which is accompanied by progressive telomere shortening ( 8 -  10).	gene_phenotype
72494	1	334642	5	NULL	NULL	0	NULL	mec1 cells	Cell		contains					telomere	Chromosome	wild type;;length of			NULL		0	NULL	NULL	NULL	gw60_molcell_11_5_1379_s_25	12769860	Telomere length is wild-type in  mec1 cells, but deleting both Tel1p and Mec1p results in the same initial overall rate of telomere shortening and eventual cellular senescence as deleting telomerase (although  tel1 mec1 cells divide for somewhat longer than  tlc1 cells)   (Chan et al., 2001  ; Ritchie et al., 1999  ).	gene_phenotype
72495	2	334642	5	NULL	NULL	0	NULL	Tel1p	GP	deletion of	shortens					telomere	Chromosome	length of			NULL		0	NULL	NULL	NULL	gw60_molcell_11_5_1379_s_25	12769860	Telomere length is wild-type in  mec1 cells, but deleting both Tel1p and Mec1p results in the same initial overall rate of telomere shortening and eventual cellular senescence as deleting telomerase (although  tel1 mec1 cells divide for somewhat longer than  tlc1 cells)   (Chan et al., 2001  ; Ritchie et al., 1999  ).	gene_phenotype
72496	3	334642	5	NULL	NULL	0	NULL	Mec1p	GP	deletion of	shortens					telomere	Chromosome	length of			NULL		0	NULL	NULL	NULL	gw60_molcell_11_5_1379_s_25	12769860	Telomere length is wild-type in  mec1 cells, but deleting both Tel1p and Mec1p results in the same initial overall rate of telomere shortening and eventual cellular senescence as deleting telomerase (although  tel1 mec1 cells divide for somewhat longer than  tlc1 cells)   (Chan et al., 2001  ; Ritchie et al., 1999  ).	gene_phenotype
72497	4	334642	5	NULL	NULL	0	NULL	statement 2	Process		leads to		eventualy			cellular senescence	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_11_5_1379_s_25	12769860	Telomere length is wild-type in  mec1 cells, but deleting both Tel1p and Mec1p results in the same initial overall rate of telomere shortening and eventual cellular senescence as deleting telomerase (although  tel1 mec1 cells divide for somewhat longer than  tlc1 cells)   (Chan et al., 2001  ; Ritchie et al., 1999  ).	gene_phenotype
72498	5	334642	5	NULL	NULL	0	NULL	statement 3	Process		leads to		eventualy			cellular senescence	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_11_5_1379_s_25	12769860	Telomere length is wild-type in  mec1 cells, but deleting both Tel1p and Mec1p results in the same initial overall rate of telomere shortening and eventual cellular senescence as deleting telomerase (although  tel1 mec1 cells divide for somewhat longer than  tlc1 cells)   (Chan et al., 2001  ; Ritchie et al., 1999  ).	gene_phenotype
72501	6	334642	5	NULL	NULL	NULL	NULL	telomerase	GP	deletion of	shortens					telomere	Chromosome	length of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_5_1379_s_25	12769860	Telomere length is wild-type in  mec1 cells, but deleting both Tel1p and Mec1p results in the same initial overall rate of telomere shortening and eventual cellular senescence as deleting telomerase (although  tel1 mec1 cells divide for somewhat longer than  tlc1 cells)   (Chan et al., 2001  ; Ritchie et al., 1999  ).	gene_phenotype
72502	7	334642	5	NULL	NULL	NULL	NULL	statement 6	Process		leads to		eventualy			cellular senescence	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_5_1379_s_25	12769860	Telomere length is wild-type in  mec1 cells, but deleting both Tel1p and Mec1p results in the same initial overall rate of telomere shortening and eventual cellular senescence as deleting telomerase (although  tel1 mec1 cells divide for somewhat longer than  tlc1 cells)   (Chan et al., 2001  ; Ritchie et al., 1999  ).	gene_phenotype
72866	1	334644	5	NULL	NULL	NULL	NULL	telomeric DNA	NucleicAcid	gradual loss of	occurs during					spore	Cell	growth of			NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_5_1379_s_151	12769860	Gradual loss of telomeric DNA during spore growth produced  tlc1 tel1 cells with an average telomere length of about 480 bp at the time they were assayed (compared to a mean length of 350 bp in wild-type cells;   Figure 3A).	gene_phenotype
72867	2	334644	5	NULL	NULL	0	NULL	tlc1 tel1 cells	Cell		contains					telomere	Chromosome	average length of			NULL		0	NULL	NULL	NULL	gw60_molcell_11_5_1379_s_151	12769860	Gradual loss of telomeric DNA during spore growth produced  tlc1 tel1 cells with an average telomere length of about 480 bp at the time they were assayed (compared to a mean length of 350 bp in wild-type cells;   Figure 3A).	gene_phenotype
72868	3	334644	5	NULL	NULL	0	NULL	statement 1	Process		produce					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_11_5_1379_s_151	12769860	Gradual loss of telomeric DNA during spore growth produced  tlc1 tel1 cells with an average telomere length of about 480 bp at the time they were assayed (compared to a mean length of 350 bp in wild-type cells;   Figure 3A).	gene_phenotype
72875	1	334646	5	NULL	NULL	0	NULL	snRNAs	NucleicAcid		is a type of					RNA polymerase II transcripts	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6046_s_23	12167699	In addition to their high uridine content, snRNAs and Tlc1 are RNA polymerase II transcripts; they have a 5''-2,2,7-trimethylguanosine (TMG) cap; and they bind the Sm proteins through a specific sequence termed the Sm site, which is essential for their accumulation ( 4,  45; snRNP biogenesis has been reviewed in reference  55).	gene_phenotype
72876	2	334646	5	NULL	NULL	0	NULL	Tlc1	NucleicAcid		is a type of					RNA polymerase II transcripts	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6046_s_23	12167699	In addition to their high uridine content, snRNAs and Tlc1 are RNA polymerase II transcripts; they have a 5''-2,2,7-trimethylguanosine (TMG) cap; and they bind the Sm proteins through a specific sequence termed the Sm site, which is essential for their accumulation ( 4,  45; snRNP biogenesis has been reviewed in reference  55).	gene_phenotype
72878	3	334646	5	NULL	NULL	0	NULL	snRNAs	NucleicAcid		contains					uridine	NucleicAcid	high			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6046_s_23	12167699	In addition to their high uridine content, snRNAs and Tlc1 are RNA polymerase II transcripts; they have a 5''-2,2,7-trimethylguanosine (TMG) cap; and they bind the Sm proteins through a specific sequence termed the Sm site, which is essential for their accumulation ( 4,  45; snRNP biogenesis has been reviewed in reference  55).	gene_phenotype
72879	4	334646	5	NULL	NULL	0	NULL	Tlc1	NucleicAcid		contains					uridine	NucleicAcid	high			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6046_s_23	12167699	In addition to their high uridine content, snRNAs and Tlc1 are RNA polymerase II transcripts; they have a 5''-2,2,7-trimethylguanosine (TMG) cap; and they bind the Sm proteins through a specific sequence termed the Sm site, which is essential for their accumulation ( 4,  45; snRNP biogenesis has been reviewed in reference  55).	gene_phenotype
72880	5	334646	5	NULL	NULL	0	NULL	TMG	NucleicAcid		is					2,2,7-trimethylguanosine	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6046_s_23	12167699	In addition to their high uridine content, snRNAs and Tlc1 are RNA polymerase II transcripts; they have a 5''-2,2,7-trimethylguanosine (TMG) cap; and they bind the Sm proteins through a specific sequence termed the Sm site, which is essential for their accumulation ( 4,  45; snRNP biogenesis has been reviewed in reference  55).	gene_phenotype
72881	6	334646	5	NULL	NULL	0	NULL	snRNAs	NucleicAcid		contains					TMG cap	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6046_s_23	12167699	In addition to their high uridine content, snRNAs and Tlc1 are RNA polymerase II transcripts; they have a 5''-2,2,7-trimethylguanosine (TMG) cap; and they bind the Sm proteins through a specific sequence termed the Sm site, which is essential for their accumulation ( 4,  45; snRNP biogenesis has been reviewed in reference  55).	gene_phenotype
72882	7	334646	5	NULL	NULL	0	NULL	Tlc1	NucleicAcid		contains					TMG cap	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6046_s_23	12167699	In addition to their high uridine content, snRNAs and Tlc1 are RNA polymerase II transcripts; they have a 5''-2,2,7-trimethylguanosine (TMG) cap; and they bind the Sm proteins through a specific sequence termed the Sm site, which is essential for their accumulation ( 4,  45; snRNP biogenesis has been reviewed in reference  55).	gene_phenotype
72883	8	334646	5	NULL	NULL	NULL	NULL	snRNAs	NucleicAcid		bind				Sm site	Sm proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6046_s_23	12167699	In addition to their high uridine content, snRNAs and Tlc1 are RNA polymerase II transcripts; they have a 5''-2,2,7-trimethylguanosine (TMG) cap; and they bind the Sm proteins through a specific sequence termed the Sm site, which is essential for their accumulation ( 4,  45; snRNP biogenesis has been reviewed in reference  55).	gene_phenotype
72884	9	334646	5	NULL	NULL	NULL	NULL	Tlc1	NucleicAcid		bind				Sm site	Sm proteins	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6046_s_23	12167699	In addition to their high uridine content, snRNAs and Tlc1 are RNA polymerase II transcripts; they have a 5''-2,2,7-trimethylguanosine (TMG) cap; and they bind the Sm proteins through a specific sequence termed the Sm site, which is essential for their accumulation ( 4,  45; snRNP biogenesis has been reviewed in reference  55).	gene_phenotype
72888	10	334646	5	NULL	NULL	NULL	NULL	snRNAs	NucleicAcid		is essential for				Sm site	snRNAs	NucleicAcid	accumulation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_17_6046_s_23	12167699	In addition to their high uridine content, snRNAs and Tlc1 are RNA polymerase II transcripts; they have a 5''-2,2,7-trimethylguanosine (TMG) cap; and they bind the Sm proteins through a specific sequence termed the Sm site, which is essential for their accumulation ( 4,  45; snRNP biogenesis has been reviewed in reference  55).	gene_phenotype
72889	11	334646	5	NULL	NULL	0	NULL	Tlc1	NucleicAcid		is essential for					Tlc1	NucleicAcid	accumulation of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6046_s_23	12167699	In addition to their high uridine content, snRNAs and Tlc1 are RNA polymerase II transcripts; they have a 5''-2,2,7-trimethylguanosine (TMG) cap; and they bind the Sm proteins through a specific sequence termed the Sm site, which is essential for their accumulation ( 4,  45; snRNP biogenesis has been reviewed in reference  55).	gene_phenotype
72890	1	334647	5	NULL	NULL	0	NULL	snRNP	GP		is a type of					small nuclear ribonucleoprotein particle	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_7_2366_s_22	11884619	In addition,  TLC1 RNA contains an Sm binding site near its 3' end that is important for the stability of the RNA and is bound by Sm proteins, therefore leading to the classification of  S. cerevisiae telomerase as an Sm snRNP (small nuclear ribonucleoprotein particle) ( 35).	gene_phenotype
72891	2	334647	5	NULL	NULL	0	NULL	TLC1 RNA	NucleicAcid		is present near				Sm binding site	TLC1 RNA	NucleicAcid			3' end	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_7_2366_s_22	11884619	In addition,  TLC1 RNA contains an Sm binding site near its 3' end that is important for the stability of the RNA and is bound by Sm proteins, therefore leading to the classification of  S. cerevisiae telomerase as an Sm snRNP (small nuclear ribonucleoprotein particle) ( 35).	gene_phenotype
72892	3	334647	5	NULL	NULL	0	NULL	statement 2	NucleicAcid		is important for					RNA	NucleicAcid	stability of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_7_2366_s_22	11884619	In addition,  TLC1 RNA contains an Sm binding site near its 3' end that is important for the stability of the RNA and is bound by Sm proteins, therefore leading to the classification of  S. cerevisiae telomerase as an Sm snRNP (small nuclear ribonucleoprotein particle) ( 35).	gene_phenotype
72893	4	334647	5	NULL	NULL	0	NULL	Sm proteins	GP		bind					TLC1 RNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_7_2366_s_22	11884619	In addition,  TLC1 RNA contains an Sm binding site near its 3' end that is important for the stability of the RNA and is bound by Sm proteins, therefore leading to the classification of  S. cerevisiae telomerase as an Sm snRNP (small nuclear ribonucleoprotein particle) ( 35).	gene_phenotype
72894	5	334647	5	NULL	NULL	0	NULL	telomerase	GP	S. cerevisiae	is classified as					snRNP	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_7_2366_s_22	11884619	In addition,  TLC1 RNA contains an Sm binding site near its 3' end that is important for the stability of the RNA and is bound by Sm proteins, therefore leading to the classification of  S. cerevisiae telomerase as an Sm snRNP (small nuclear ribonucleoprotein particle) ( 35).	gene_phenotype
72895	1	334648	5	NULL	NULL	0	NULL	CP motif	AminoAcid	mutation of	reduce					TERT protein	GP	amount of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_6_3882_s_143	12458198	Mutations in the CP, QFP, and T Motifs Caused a Reduction in the Amount of TERT Protein and TERT-associated TLC1 RNA-- To determine the basis for the activity loss manifested by the SCR mutants, we estimated the levels of TERT protein in wild type and mutant strains using antibodies directed against the protein A tag.	gene_phenotype
72896	2	334648	5	NULL	NULL	0	NULL	QFP motif	AminoAcid	mutation of	reduce					TERT protein	GP	amount of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_6_3882_s_143	12458198	Mutations in the CP, QFP, and T Motifs Caused a Reduction in the Amount of TERT Protein and TERT-associated TLC1 RNA-- To determine the basis for the activity loss manifested by the SCR mutants, we estimated the levels of TERT protein in wild type and mutant strains using antibodies directed against the protein A tag.	gene_phenotype
72897	3	334648	5	NULL	NULL	0	NULL	T Motif	AminoAcid	mutation of	reduce					TERT protein	GP	amount of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_6_3882_s_143	12458198	Mutations in the CP, QFP, and T Motifs Caused a Reduction in the Amount of TERT Protein and TERT-associated TLC1 RNA-- To determine the basis for the activity loss manifested by the SCR mutants, we estimated the levels of TERT protein in wild type and mutant strains using antibodies directed against the protein A tag.	gene_phenotype
72898	4	334648	5	NULL	NULL	0	NULL	TLC1 RNA	NucleicAcid		associates with					TERT	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_6_3882_s_143	12458198	Mutations in the CP, QFP, and T Motifs Caused a Reduction in the Amount of TERT Protein and TERT-associated TLC1 RNA-- To determine the basis for the activity loss manifested by the SCR mutants, we estimated the levels of TERT protein in wild type and mutant strains using antibodies directed against the protein A tag.	gene_phenotype
72899	5	334648	5	NULL	NULL	0	NULL	CP motif	AminoAcid	mutation of	reduce					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_6_3882_s_143	12458198	Mutations in the CP, QFP, and T Motifs Caused a Reduction in the Amount of TERT Protein and TERT-associated TLC1 RNA-- To determine the basis for the activity loss manifested by the SCR mutants, we estimated the levels of TERT protein in wild type and mutant strains using antibodies directed against the protein A tag.	gene_phenotype
72900	6	334648	5	NULL	NULL	0	NULL	QFP motif	AminoAcid	mutation of	reduce					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_6_3882_s_143	12458198	Mutations in the CP, QFP, and T Motifs Caused a Reduction in the Amount of TERT Protein and TERT-associated TLC1 RNA-- To determine the basis for the activity loss manifested by the SCR mutants, we estimated the levels of TERT protein in wild type and mutant strains using antibodies directed against the protein A tag.	gene_phenotype
72901	7	334648	5	NULL	NULL	0	NULL	T Motif	AminoAcid	mutation of	reduce					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_6_3882_s_143	12458198	Mutations in the CP, QFP, and T Motifs Caused a Reduction in the Amount of TERT Protein and TERT-associated TLC1 RNA-- To determine the basis for the activity loss manifested by the SCR mutants, we estimated the levels of TERT protein in wild type and mutant strains using antibodies directed against the protein A tag.	gene_phenotype
72902	1	334651	5	NULL	NULL	0	NULL	telomerase	GP		adds					repeats	NucleicAcid	new			NULL		0	NULL	NULL	NULL	gw60_pnas_97_21_11409_s_256	11016977	Concurrent disruption of both the ability of telomerase to add new repeats and the ability of those repeats to negatively regulate telomere length might explain the simultaneously existing populations of elongated and shortened telomeres exhibited initially by certain  ter1 and  tlc1 template mutants (this work and ref.  14).	gene_phenotype
73060	2	334651	5	NULL	NULL	0	NULL	repeats	NucleicAcid	newly added	regulate		negatively			telomere	Chromosome	length of			NULL		0	NULL	NULL	NULL	gw60_pnas_97_21_11409_s_256	11016977	Concurrent disruption of both the ability of telomerase to add new repeats and the ability of those repeats to negatively regulate telomere length might explain the simultaneously existing populations of elongated and shortened telomeres exhibited initially by certain  ter1 and  tlc1 template mutants (this work and ref.  14).	gene_phenotype
73061	3	334651	5	NULL	NULL	0	NULL	telomere	Chromosome	elongated	exists with		simultaneously			telomere	Chromosome	shortened			NULL	ter1 template mutants	0	NULL	NULL	NULL	gw60_pnas_97_21_11409_s_256	11016977	Concurrent disruption of both the ability of telomerase to add new repeats and the ability of those repeats to negatively regulate telomere length might explain the simultaneously existing populations of elongated and shortened telomeres exhibited initially by certain  ter1 and  tlc1 template mutants (this work and ref.  14).	gene_phenotype
73062	4	334651	5	NULL	NULL	0	NULL	telomere	Chromosome	elongated	exists with		simultaneously			telomere	Chromosome	shortened			NULL	tlc1 template mutants	0	NULL	NULL	NULL	gw60_pnas_97_21_11409_s_256	11016977	Concurrent disruption of both the ability of telomerase to add new repeats and the ability of those repeats to negatively regulate telomere length might explain the simultaneously existing populations of elongated and shortened telomeres exhibited initially by certain  ter1 and  tlc1 template mutants (this work and ref.  14).	gene_phenotype
73063	5	334651	5	NULL	NULL	NULL	NULL	statement 1	Process		is disrupted with		concurrently			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11409_s_256	11016977	Concurrent disruption of both the ability of telomerase to add new repeats and the ability of those repeats to negatively regulate telomere length might explain the simultaneously existing populations of elongated and shortened telomeres exhibited initially by certain  ter1 and  tlc1 template mutants (this work and ref.  14).	gene_phenotype
73064	6	334651	5	NULL	NULL	NULL	NULL	statement 5	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11409_s_256	11016977	Concurrent disruption of both the ability of telomerase to add new repeats and the ability of those repeats to negatively regulate telomere length might explain the simultaneously existing populations of elongated and shortened telomeres exhibited initially by certain  ter1 and  tlc1 template mutants (this work and ref.  14).	gene_phenotype
73065	7	334651	5	NULL	NULL	NULL	NULL	statement 5	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11409_s_256	11016977	Concurrent disruption of both the ability of telomerase to add new repeats and the ability of those repeats to negatively regulate telomere length might explain the simultaneously existing populations of elongated and shortened telomeres exhibited initially by certain  ter1 and  tlc1 template mutants (this work and ref.  14).	gene_phenotype
73066	1	334655	5	NULL	NULL	0	NULL	telomere	Chromosome	shortening of	is followed by					viability	Process	progressive loss of			NULL		0	NULL	NULL	NULL	gw60_genesdev_12_8_1073_s_136	9553037	Strains carrying deletions of  EST1, EST2, EST3, or  TLC1 exhibit the in vivo phenotypes predicted for a telomerase defect (telomere shortening and progressive loss of viability, termed yeast cellular senescence), and epistasis tests have shown that these four genes act in a single pathway for telomere replication (Lundblad and Szostak 1989  ; Lendvay et al. 1996  ; Lingner et al. 1997b  ).	gene_phenotype
73067	2	334655	5	NULL	NULL	0	NULL	statement 1	Process		is termed as					yeast cellular senescence	Process				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_8_1073_s_136	9553037	Strains carrying deletions of  EST1, EST2, EST3, or  TLC1 exhibit the in vivo phenotypes predicted for a telomerase defect (telomere shortening and progressive loss of viability, termed yeast cellular senescence), and epistasis tests have shown that these four genes act in a single pathway for telomere replication (Lundblad and Szostak 1989  ; Lendvay et al. 1996  ; Lingner et al. 1997b  ).	gene_phenotype
73068	3	334655	5	NULL	NULL	0	NULL	yeast cellular senescence	Process		is a type of					telomerase defect	Process				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_8_1073_s_136	9553037	Strains carrying deletions of  EST1, EST2, EST3, or  TLC1 exhibit the in vivo phenotypes predicted for a telomerase defect (telomere shortening and progressive loss of viability, termed yeast cellular senescence), and epistasis tests have shown that these four genes act in a single pathway for telomere replication (Lundblad and Szostak 1989  ; Lendvay et al. 1996  ; Lingner et al. 1997b  ).	gene_phenotype
73069	4	334655	5	NULL	NULL	0	NULL	EST1	GP	deletion of	leads to					yeast cellular senescence	Process				NULL	in vivo	0	NULL	NULL	NULL	gw60_genesdev_12_8_1073_s_136	9553037	Strains carrying deletions of  EST1, EST2, EST3, or  TLC1 exhibit the in vivo phenotypes predicted for a telomerase defect (telomere shortening and progressive loss of viability, termed yeast cellular senescence), and epistasis tests have shown that these four genes act in a single pathway for telomere replication (Lundblad and Szostak 1989  ; Lendvay et al. 1996  ; Lingner et al. 1997b  ).	gene_phenotype
73070	5	334655	5	NULL	NULL	0	NULL	EST2	GP	deletion of	leads to					yeast cellular senescence	Process				NULL	in vivo	0	NULL	NULL	NULL	gw60_genesdev_12_8_1073_s_136	9553037	Strains carrying deletions of  EST1, EST2, EST3, or  TLC1 exhibit the in vivo phenotypes predicted for a telomerase defect (telomere shortening and progressive loss of viability, termed yeast cellular senescence), and epistasis tests have shown that these four genes act in a single pathway for telomere replication (Lundblad and Szostak 1989  ; Lendvay et al. 1996  ; Lingner et al. 1997b  ).	gene_phenotype
73071	6	334655	5	NULL	NULL	0	NULL	EST3	GP	deletion of	leads to					yeast cellular senescence	Process				NULL	in vivo	0	NULL	NULL	NULL	gw60_genesdev_12_8_1073_s_136	9553037	Strains carrying deletions of  EST1, EST2, EST3, or  TLC1 exhibit the in vivo phenotypes predicted for a telomerase defect (telomere shortening and progressive loss of viability, termed yeast cellular senescence), and epistasis tests have shown that these four genes act in a single pathway for telomere replication (Lundblad and Szostak 1989  ; Lendvay et al. 1996  ; Lingner et al. 1997b  ).	gene_phenotype
73072	7	334655	5	NULL	NULL	0	NULL	TLC1	GP	deletion of	leads to					yeast cellular senescence	Process				NULL	in vivo	0	NULL	NULL	NULL	gw60_genesdev_12_8_1073_s_136	9553037	Strains carrying deletions of  EST1, EST2, EST3, or  TLC1 exhibit the in vivo phenotypes predicted for a telomerase defect (telomere shortening and progressive loss of viability, termed yeast cellular senescence), and epistasis tests have shown that these four genes act in a single pathway for telomere replication (Lundblad and Szostak 1989  ; Lendvay et al. 1996  ; Lingner et al. 1997b  ).	gene_phenotype
73073	8	334655	5	NULL	NULL	0	NULL	EST1 gene	GP		plays a role in					telomere	Chromosome	replication of			NULL		0	NULL	NULL	NULL	gw60_genesdev_12_8_1073_s_136	9553037	Strains carrying deletions of  EST1, EST2, EST3, or  TLC1 exhibit the in vivo phenotypes predicted for a telomerase defect (telomere shortening and progressive loss of viability, termed yeast cellular senescence), and epistasis tests have shown that these four genes act in a single pathway for telomere replication (Lundblad and Szostak 1989  ; Lendvay et al. 1996  ; Lingner et al. 1997b  ).	gene_phenotype
73074	9	334655	5	NULL	NULL	0	NULL	EST2 gene	GP		plays a role in					telomere	Chromosome	replication of			NULL		0	NULL	NULL	NULL	gw60_genesdev_12_8_1073_s_136	9553037	Strains carrying deletions of  EST1, EST2, EST3, or  TLC1 exhibit the in vivo phenotypes predicted for a telomerase defect (telomere shortening and progressive loss of viability, termed yeast cellular senescence), and epistasis tests have shown that these four genes act in a single pathway for telomere replication (Lundblad and Szostak 1989  ; Lendvay et al. 1996  ; Lingner et al. 1997b  ).	gene_phenotype
73075	10	334655	5	NULL	NULL	0	NULL	EST3 gene	GP		plays a role in					telomere	Chromosome	replication of			NULL		0	NULL	NULL	NULL	gw60_genesdev_12_8_1073_s_136	9553037	Strains carrying deletions of  EST1, EST2, EST3, or  TLC1 exhibit the in vivo phenotypes predicted for a telomerase defect (telomere shortening and progressive loss of viability, termed yeast cellular senescence), and epistasis tests have shown that these four genes act in a single pathway for telomere replication (Lundblad and Szostak 1989  ; Lendvay et al. 1996  ; Lingner et al. 1997b  ).	gene_phenotype
73076	11	334655	5	NULL	NULL	0	NULL	TLC1 gene	GP		plays a role in					telomere	Chromosome	replication of			NULL		0	NULL	NULL	NULL	gw60_genesdev_12_8_1073_s_136	9553037	Strains carrying deletions of  EST1, EST2, EST3, or  TLC1 exhibit the in vivo phenotypes predicted for a telomerase defect (telomere shortening and progressive loss of viability, termed yeast cellular senescence), and epistasis tests have shown that these four genes act in a single pathway for telomere replication (Lundblad and Szostak 1989  ; Lendvay et al. 1996  ; Lingner et al. 1997b  ).	gene_phenotype
73077	1	334656	5	NULL	NULL	0	NULL	DOT genes	GP		maintain		may			telomeric DNA	NucleicAcid	normal structure of			NULL		0	NULL	NULL	NULL	gw60_genetics_150_2_613_s_406	9755194	Effects of deleting the  DOT genes on telomeric DNA tract length:   Finally, to assess whether the  DOT genes have a role in maintaining normal telomeric DNA structure, telomere length was measured using a TG1-3 probe that detected all telomeres in the cell in strains deleted for one of the nonessential genes isolated in the screen [ DOT1,  DOT4,  DOT5,  DOT6,  ASF1, and  SIR4 ( TLC1 results were published earlier in   S INGER and GOTTSCHLING 1994   )].	gene_phenotype
73078	1	334657	5	NULL	NULL	0	NULL	tlc1-h cells	Cell		is a synonym of					humanized yeast	Cell				NULL		0	NULL	NULL	NULL	gw70_embo_25_4_846_s_38	16467854	In  tlc1-h cells, also known as humanized yeast (  et al), a telomere formed only by vertebrate repeats can be maintained at a regulated mean  length ( ;   et al).	gene_phenotype
73079	2	334657	5	NULL	NULL	NULL	NULL	telomere	Chromosome		is formed by		only			repeats	NucleicAcid	vertebrate			NULL	humanized yeast	NULL	NULL	NULL	NULL	gw70_embo_25_4_846_s_38	16467854	In  tlc1-h cells, also known as humanized yeast (  et al), a telomere formed only by vertebrate repeats can be maintained at a regulated mean  length ( ;   et al).	gene_phenotype
73080	1	334658	5	NULL	NULL	0	NULL	repeats	NucleicAcid	vertebrate	regulates					telomere	Chromosome	length of			NULL		0	NULL	NULL	NULL	gw70_embo_25_4_846_s_39	16467854	It is noteworthy that, in  tlc1-h cells containing a functional  TEL1 gene, the number of vertebrate repeats at a chromosome end is determined in a Rap1-independent  manner, indicating that  TEL1 does not completely abolish the ability of vertebrate repeats to regulate telomere  length.	gene_phenotype
73081	2	334658	5	NULL	NULL	0	NULL	TEL1	GP		does not abolish		completely			statement 1	Process				NULL	tlc1-h cells	0	NULL	NULL	NULL	gw70_embo_25_4_846_s_39	16467854	It is noteworthy that, in  tlc1-h cells containing a functional  TEL1 gene, the number of vertebrate repeats at a chromosome end is determined in a Rap1-independent  manner, indicating that  TEL1 does not completely abolish the ability of vertebrate repeats to regulate telomere  length.	gene_phenotype
73082	3	334658	5	NULL	NULL	0	NULL	tlc1-h cells	Cell		contains					TEL1 gene	GP	functional			NULL		0	NULL	NULL	NULL	gw70_embo_25_4_846_s_39	16467854	It is noteworthy that, in  tlc1-h cells containing a functional  TEL1 gene, the number of vertebrate repeats at a chromosome end is determined in a Rap1-independent  manner, indicating that  TEL1 does not completely abolish the ability of vertebrate repeats to regulate telomere  length.	gene_phenotype
73083	1	334659	5	NULL	NULL	0	NULL	tlc1-h cells	Cell		is a synonym of					humanized yeast	Cell				NULL		0	NULL	NULL	NULL	gw70_embo_22_7_1697_s_184	12660175	In  tlc1-h cells, also known as humanized yeast (  et al), a T2AG3-only telomere formed only by vertebrate repeats can be maintained at a regulated  mean length ( Figure 5B).	gene_phenotype
73084	2	334659	5	NULL	NULL	0	NULL	T2AG3-only telomere	Chromosome		is formed by		only			repeats	NucleicAcid	vertebrate			NULL	humanized yeast\t\t	0	NULL	NULL	NULL	gw70_embo_22_7_1697_s_184	12660175	In  tlc1-h cells, also known as humanized yeast (  et al), a T2AG3-only telomere formed only by vertebrate repeats can be maintained at a regulated  mean length ( Figure 5B).	gene_phenotype
73085	1	334663	5	NULL	NULL	0	NULL	Campylobacter pyloridis	OrganismPart		is associated with					intercellular spaces	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_18_5274_s_172	10960117	Campylobacter pyloridis and gastritis: association with intercellular spaces and adaptation to an environment of mucus as important factors in colonization of the gastric epithelium.	gene_phenotype
73086	2	334663	5	NULL	NULL	0	NULL	statement 1	Process		plays a role in		important			gastric epithelium	Cell	colonization of			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_18_5274_s_172	10960117	Campylobacter pyloridis and gastritis: association with intercellular spaces and adaptation to an environment of mucus as important factors in colonization of the gastric epithelium.	gene_phenotype
73087	3	334663	5	NULL	NULL	NULL	NULL	Campylobacter pyloridis	Organism		is adapted to					mucus 	Chemical	environment of			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_18_5274_s_172	10960117	Campylobacter pyloridis and gastritis: association with intercellular spaces and adaptation to an environment of mucus as important factors in colonization of the gastric epithelium.	gene_phenotype
73088	4	334663	5	NULL	NULL	0	NULL	statement 3	Process		plays a role in		important			gastric epithelium	Cell	colonization of			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_18_5274_s_172	10960117	Campylobacter pyloridis and gastritis: association with intercellular spaces and adaptation to an environment of mucus as important factors in colonization of the gastric epithelium.	gene_phenotype
73089	5	334663	5	NULL	NULL	0	NULL	gastritis	MedicalFinding		is associated with					intercellular spaces	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_18_5274_s_172	10960117	Campylobacter pyloridis and gastritis: association with intercellular spaces and adaptation to an environment of mucus as important factors in colonization of the gastric epithelium.	gene_phenotype
73090	6	334663	5	NULL	NULL	0	NULL	statement 5	Process		plays a role in		important			gastric epithelium	Cell	colonization of			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_18_5274_s_172	10960117	Campylobacter pyloridis and gastritis: association with intercellular spaces and adaptation to an environment of mucus as important factors in colonization of the gastric epithelium.	gene_phenotype
73091	7	334663	5	NULL	NULL	NULL	NULL	gastritis	MedicalFinding		is adapted to					mucus	Chemical	environment of			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_182_18_5274_s_172	10960117	Campylobacter pyloridis and gastritis: association with intercellular spaces and adaptation to an environment of mucus as important factors in colonization of the gastric epithelium.	gene_phenotype
73092	8	334663	5	NULL	NULL	0	NULL	statement 7	Process		plays a role in		important			gastric epithelium	Cell	colonization of			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_18_5274_s_172	10960117	Campylobacter pyloridis and gastritis: association with intercellular spaces and adaptation to an environment of mucus as important factors in colonization of the gastric epithelium.	gene_phenotype
73093	1	334665	5	NULL	NULL	0	NULL	LPS	Chemical		induce					IkappaB	GP	phosphorylation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_11_10776_s_219	14679201	D, NO inhibits LPS-induced IkappaB phosphorylation.	gene_phenotype
73094	2	334665	5	NULL	NULL	0	NULL	NO	Chemical		inhibits					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_11_10776_s_219	14679201	D, NO inhibits LPS-induced IkappaB phosphorylation.	gene_phenotype
73095	1	334667	5	NULL	NULL	0	NULL	suppressive petites	NucleicAcid		is a dominant deletion mutant of					mtDNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_pnas_94_23_12503_s_73	9356479	Suppressive petites, for example, are dominant deletion mutants of mtDNA, which depend, like mtDNA itself, on chromosomal genes (e.g.,  PET18), for their replication.	gene_phenotype
73096	2	334667	5	NULL	NULL	0	NULL	statement 1	Process	replication of	is dependent on					 PET18	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_94_23_12503_s_73	9356479	Suppressive petites, for example, are dominant deletion mutants of mtDNA, which depend, like mtDNA itself, on chromosomal genes (e.g.,  PET18), for their replication.	gene_phenotype
73097	3	334667	5	NULL	NULL	0	NULL	 PET18	GP		is a type of					chromosomal gene	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_94_23_12503_s_73	9356479	Suppressive petites, for example, are dominant deletion mutants of mtDNA, which depend, like mtDNA itself, on chromosomal genes (e.g.,  PET18), for their replication.	gene_phenotype
73098	4	334667	5	NULL	NULL	0	NULL	mtDNA	NucleicAcid	replication of	is dependent on					PET18	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_94_23_12503_s_73	9356479	Suppressive petites, for example, are dominant deletion mutants of mtDNA, which depend, like mtDNA itself, on chromosomal genes (e.g.,  PET18), for their replication.	gene_phenotype
73099	1	334668	5	NULL	NULL	0	NULL	PET111	GP	null mutation;;S. kluyveri	prevents					respiratory growth	Process				NULL	nonfermentable carbon source	0	NULL	NULL	NULL	gw60_genetics_154_3_999_s_238	10757749	These null mutations in  S. kluyveri PET111,  K. lactis PET111, or  S. kluyveri PET122 all prevented respiratory growth on nonfermentable carbon sources.	gene_phenotype
73100	2	334668	5	NULL	NULL	0	NULL	PET111	GP	null mutant;;K. lactis	prevents					respiratory growth	Process				NULL	nonfermentable carbon source	0	NULL	NULL	NULL	gw60_genetics_154_3_999_s_238	10757749	These null mutations in  S. kluyveri PET111,  K. lactis PET111, or  S. kluyveri PET122 all prevented respiratory growth on nonfermentable carbon sources.	gene_phenotype
73101	3	334668	5	NULL	NULL	0	NULL	PET122	GP	null mutant;;S. kluyveri	prevents					respiratory growth	Process				NULL	nonfermentable carbon source	0	NULL	NULL	NULL	gw60_genetics_154_3_999_s_238	10757749	These null mutations in  S. kluyveri PET111,  K. lactis PET111, or  S. kluyveri PET122 all prevented respiratory growth on nonfermentable carbon sources.	gene_phenotype
73102	1	334672	5	NULL	NULL	0	NULL	pet18 gene	GP	mutant	confer					respire	Process	inability to			NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	abs-batch0650-0679_mol-gen-genet_165_2_366371_s_2	366371	Mutations in the pet18 gene of Saccharomyces cerevisiae (formerly denoted  pets) confer three phenotypes on mutant strains: (i) inability to respire  (petite), (ii) inability to maintain the double-stranded RNA killer plasmid  (sensitive), and (iii) temperature sensitivity for growth.	gene_phenotype
73103	2	334672	5	NULL	NULL	NULL	NULL	pet18 gene	GP	mutant	confer					double-stranded RNA killer plasmid	CellComponent	inability to maintain			NULL	Saccharomyces cerevisiae	NULL	NULL	NULL	NULL	abs-batch0650-0679_mol-gen-genet_165_2_366371_s_2	366371	Mutations in the pet18 gene of Saccharomyces cerevisiae (formerly denoted  pets) confer three phenotypes on mutant strains: (i) inability to respire  (petite), (ii) inability to maintain the double-stranded RNA killer plasmid  (sensitive), and (iii) temperature sensitivity for growth.	gene_phenotype
73104	3	334672	5	NULL	NULL	0	NULL	pet18 gene	GP	mutant	confer					growth	Process	temperature sensitivity of			NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	abs-batch0650-0679_mol-gen-genet_165_2_366371_s_2	366371	Mutations in the pet18 gene of Saccharomyces cerevisiae (formerly denoted  pets) confer three phenotypes on mutant strains: (i) inability to respire  (petite), (ii) inability to maintain the double-stranded RNA killer plasmid  (sensitive), and (iii) temperature sensitivity for growth.	gene_phenotype
73105	1	334674	5	NULL	NULL	0	NULL	axoplasmic transport	Process		is required for					AR	GP	 normal expression of			NULL		0	NULL	NULL	NULL	gw60_pnas_94_4_1521_s_136	9037086	Thus, axoplasmic transport is required for normal expression of AR.	gene_phenotype
73141	1	334680	5	NULL	NULL	0	NULL	ascii	Cell		contains					respiratory growth-deficient spore	Cell				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_24_16305_s_98	16608846	As expected, the ascii usually contained two spores, both respiratory growth-deficient and leucine-prototrophic, as a result of the  pet111 deletion (not shown).	gene_phenotype
73142	2	334680	5	NULL	NULL	0	NULL	ascii	Cell		contains					leucine-prototrophic spore	Cell				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_24_16305_s_98	16608846	As expected, the ascii usually contained two spores, both respiratory growth-deficient and leucine-prototrophic, as a result of the  pet111 deletion (not shown).	gene_phenotype
73143	3	334680	5	NULL	NULL	0	NULL	pet111	GP	deletion of	leads to					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_24_16305_s_98	16608846	As expected, the ascii usually contained two spores, both respiratory growth-deficient and leucine-prototrophic, as a result of the  pet111 deletion (not shown).	gene_phenotype
73144	4	334680	5	NULL	NULL	0	NULL	pet111	GP	deletion of	leads to					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_24_16305_s_98	16608846	As expected, the ascii usually contained two spores, both respiratory growth-deficient and leucine-prototrophic, as a result of the  pet111 deletion (not shown).	gene_phenotype
73145	1	334682	5	NULL	NULL	0	NULL	cox2-11 strain	Cell		contains					suppressor	AbstractConcept				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_4_1826_s_96	9528754	Respiratory growth of the  cox2-11 strains containing these suppressors remained dependent upon the function of the  PET111 gene.	gene_phenotype
73146	2	334682	5	NULL	NULL	0	NULL	statement 1	Cell	respiratory growth of	is dependent on					 PET111 gene	GP	function of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_4_1826_s_96	9528754	Respiratory growth of the  cox2-11 strains containing these suppressors remained dependent upon the function of the  PET111 gene.	gene_phenotype
73147	1	334683	5	NULL	NULL	0	NULL	JM109(DE3)(pLysS) cells	Cell		harbor					pET11d- uxuR vector	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_12_3695_s_204	10368143	Indeed, JM109(DE3)(pLysS) cells harboring the pET11d- uxuR vector were viable and permitted low-level expression of UxuR.	gene_phenotype
73148	2	334683	5	NULL	NULL	0	NULL	UxuR	GP		is expressed in		low			statement 1	Cell				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_12_3695_s_204	10368143	Indeed, JM109(DE3)(pLysS) cells harboring the pET11d- uxuR vector were viable and permitted low-level expression of UxuR.	gene_phenotype
73149	1	334695	5	NULL	NULL	0	NULL	 CBT1	GP	deletion of	accumulates					15S RNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_genetics_171_3_949_s_140	16118200	Deletion of  CBT1 results in accumulation of 15S and  RPM1 RNAs with unprocessed 5' ends:   The defect in 5' processing of  COB in the  cbt1 deletion strains is similar to that previously shown for  pet127 mutants ( IESENBERGERand F 1997), although it is not as pronounced.	gene_phenotype
73150	2	334695	5	NULL	NULL	0	NULL	15S RNA	NucleicAcid		contains					5' ends	NucleicAcid	unprocessed			NULL		0	NULL	NULL	NULL	gw70_genetics_171_3_949_s_140	16118200	Deletion of  CBT1 results in accumulation of 15S and  RPM1 RNAs with unprocessed 5' ends:   The defect in 5' processing of  COB in the  cbt1 deletion strains is similar to that previously shown for  pet127 mutants ( IESENBERGERand F 1997), although it is not as pronounced.	gene_phenotype
73151	3	334695	5	NULL	NULL	0	NULL	 CBT1	GP	deletion of	accumulates					RPM1 RNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_genetics_171_3_949_s_140	16118200	Deletion of  CBT1 results in accumulation of 15S and  RPM1 RNAs with unprocessed 5' ends:   The defect in 5' processing of  COB in the  cbt1 deletion strains is similar to that previously shown for  pet127 mutants ( IESENBERGERand F 1997), although it is not as pronounced.	gene_phenotype
73152	4	334695	5	NULL	NULL	0	NULL	RPM1 RNA	NucleicAcid		contains					5' ends	NucleicAcid	unprocessed			NULL		0	NULL	NULL	NULL	gw70_genetics_171_3_949_s_140	16118200	Deletion of  CBT1 results in accumulation of 15S and  RPM1 RNAs with unprocessed 5' ends:   The defect in 5' processing of  COB in the  cbt1 deletion strains is similar to that previously shown for  pet127 mutants ( IESENBERGERand F 1997), although it is not as pronounced.	gene_phenotype
73153	1	334696	5	NULL	NULL	0	NULL	pet127	GP	mutation of	supress					ACG	NucleicAcid	respiratory deficiency of;;mutant			NULL		0	NULL	NULL	NULL	gw60_genetics_151_4_1315_s_219	10101159	The  pet127 mutation did suppress the respiratory deficiency of the ACG and CCU mutants and allowed very slow growth of the CAG mutant at 30 degrees  (observed after 7 days of incubation).	gene_phenotype
73154	2	334696	5	NULL	NULL	NULL	NULL	pet127	GP	mutation of	supress					CCU	NucleicAcid	respiratory deficiency of;;mutant			NULL		NULL	NULL	NULL	NULL	gw60_genetics_151_4_1315_s_219	10101159	The  pet127 mutation did suppress the respiratory deficiency of the ACG and CCU mutants and allowed very slow growth of the CAG mutant at 30 degrees  (observed after 7 days of incubation).	gene_phenotype
73155	3	334696	5	NULL	NULL	0	NULL	pet127	GP	mutation of	allows					CAG	NucleicAcid	very slow growth of;;mutant			NULL		0	NULL	NULL	NULL	gw60_genetics_151_4_1315_s_219	10101159	The  pet127 mutation did suppress the respiratory deficiency of the ACG and CCU mutants and allowed very slow growth of the CAG mutant at 30 degrees  (observed after 7 days of incubation).	gene_phenotype
73156	1	334714	5	NULL	NULL	0	NULL	 PET127 gene product	GP		is involved in					RNA	NucleicAcid	metabolism of;;mitochondrial			NULL		0	NULL	NULL	NULL	gw70_genetics_171_3_949_s_70	16118200	Suppressors of the temperature-sensitive respiratory growth phenotype of strains with the CCG triplet mutated to CC U or  ACG have been linked ( HEN et al) to the  PET127 and  DSS1 genes, which encode products involved in mitochondrial RNA metabolism ( IESENBERGEROX;  ZIEMBOWSKI et al ).	gene_phenotype
73157	2	334714	5	NULL	NULL	0	NULL	DSS1 gene product	GP		is involved in					RNA	NucleicAcid	metabolism of;;mitochondrial			NULL		0	NULL	NULL	NULL	gw70_genetics_171_3_949_s_70	16118200	Suppressors of the temperature-sensitive respiratory growth phenotype of strains with the CCG triplet mutated to CC U or  ACG have been linked ( HEN et al) to the  PET127 and  DSS1 genes, which encode products involved in mitochondrial RNA metabolism ( IESENBERGEROX;  ZIEMBOWSKI et al ).	gene_phenotype
73158	1	334730	5	NULL	NULL	0	NULL	AFP1	GP	 E. coli BL21(DE3) cell extracts	causes					antifungal activity	Process				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_24_7421_s_260	10601197	As antifungal activity has also been demonstrated for AFP1 isolated to homogeneity from  E. coli BL21(DE3) cell extracts carrying the portion of the  afp1 gene for the mature AFP1 protein in the T7 RNA polymerase-based pET11a (data not shown), there is no doubt that antifungal activity is caused by AFP1 alone.	gene_phenotype
73228	1	334764	5	NULL	NULL	0	NULL	pet20- strain	Cell		is sensitive to					calcium chloride	Chemical				NULL		0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_282	16491469	In addition to the lower cytochrome  c level and diminished growth on YPG, the  pet20-  strain was sensitive to a number of mitochondria-specific drugs, such as: calcium  chloride, which regulates mitochondrial function; oligomycin, an inhibitor of ATP  synthase and oxidative phosphorylation; potassium ferricyanide, an inhibitor of oxidative  phosphorylation; and hydrogen peroxide, a strong oxidant and stress agent that affects  proton/electron balance in the cell (Figure  2B).	gene_phenotype
73229	2	334764	5	NULL	NULL	0	NULL	calcium chloride	Chemical		is a type of					mitochondria-specific drug	Chemical				NULL		0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_282	16491469	In addition to the lower cytochrome  c level and diminished growth on YPG, the  pet20-  strain was sensitive to a number of mitochondria-specific drugs, such as: calcium  chloride, which regulates mitochondrial function; oligomycin, an inhibitor of ATP  synthase and oxidative phosphorylation; potassium ferricyanide, an inhibitor of oxidative  phosphorylation; and hydrogen peroxide, a strong oxidant and stress agent that affects  proton/electron balance in the cell (Figure  2B).	gene_phenotype
73230	3	334764	5	NULL	NULL	0	NULL	calcium chloride	Chemical		regulates					mitochondria	CellComponent	function of			NULL		0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_282	16491469	In addition to the lower cytochrome  c level and diminished growth on YPG, the  pet20-  strain was sensitive to a number of mitochondria-specific drugs, such as: calcium  chloride, which regulates mitochondrial function; oligomycin, an inhibitor of ATP  synthase and oxidative phosphorylation; potassium ferricyanide, an inhibitor of oxidative  phosphorylation; and hydrogen peroxide, a strong oxidant and stress agent that affects  proton/electron balance in the cell (Figure  2B).	gene_phenotype
73231	4	334764	5	NULL	NULL	0	NULL	pet20- strain	Cell		is sensitive to					oligomycin	Chemical				NULL		0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_282	16491469	In addition to the lower cytochrome  c level and diminished growth on YPG, the  pet20-  strain was sensitive to a number of mitochondria-specific drugs, such as: calcium  chloride, which regulates mitochondrial function; oligomycin, an inhibitor of ATP  synthase and oxidative phosphorylation; potassium ferricyanide, an inhibitor of oxidative  phosphorylation; and hydrogen peroxide, a strong oxidant and stress agent that affects  proton/electron balance in the cell (Figure  2B).	gene_phenotype
73232	5	334764	5	NULL	NULL	0	NULL	oligomycin	Chemical		is a type of					mitochondria-specific drug	Chemical				NULL		0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_282	16491469	In addition to the lower cytochrome  c level and diminished growth on YPG, the  pet20-  strain was sensitive to a number of mitochondria-specific drugs, such as: calcium  chloride, which regulates mitochondrial function; oligomycin, an inhibitor of ATP  synthase and oxidative phosphorylation; potassium ferricyanide, an inhibitor of oxidative  phosphorylation; and hydrogen peroxide, a strong oxidant and stress agent that affects  proton/electron balance in the cell (Figure  2B).	gene_phenotype
73233	6	334764	5	NULL	NULL	0	NULL	oligomycin	Chemical		is an inhibitor of					ATP synthase	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_282	16491469	In addition to the lower cytochrome  c level and diminished growth on YPG, the  pet20-  strain was sensitive to a number of mitochondria-specific drugs, such as: calcium  chloride, which regulates mitochondrial function; oligomycin, an inhibitor of ATP  synthase and oxidative phosphorylation; potassium ferricyanide, an inhibitor of oxidative  phosphorylation; and hydrogen peroxide, a strong oxidant and stress agent that affects  proton/electron balance in the cell (Figure  2B).	gene_phenotype
73235	7	334764	5	NULL	NULL	0	NULL	oligomycin	Chemical		is an inhibitor of					oxidative phosphorylation	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_282	16491469	In addition to the lower cytochrome  c level and diminished growth on YPG, the  pet20-  strain was sensitive to a number of mitochondria-specific drugs, such as: calcium  chloride, which regulates mitochondrial function; oligomycin, an inhibitor of ATP  synthase and oxidative phosphorylation; potassium ferricyanide, an inhibitor of oxidative  phosphorylation; and hydrogen peroxide, a strong oxidant and stress agent that affects  proton/electron balance in the cell (Figure  2B).	gene_phenotype
73237	8	334764	5	NULL	NULL	0	NULL	pet20- strain	Cell		is sensitive to					potassium ferricyanide	Chemical				NULL		0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_282	16491469	In addition to the lower cytochrome  c level and diminished growth on YPG, the  pet20-  strain was sensitive to a number of mitochondria-specific drugs, such as: calcium  chloride, which regulates mitochondrial function; oligomycin, an inhibitor of ATP  synthase and oxidative phosphorylation; potassium ferricyanide, an inhibitor of oxidative  phosphorylation; and hydrogen peroxide, a strong oxidant and stress agent that affects  proton/electron balance in the cell (Figure  2B).	gene_phenotype
73238	9	334764	5	NULL	NULL	0	NULL	potassium ferricyanide	Chemical		is a type of					mitochondria-specific drug	Chemical				NULL		0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_282	16491469	In addition to the lower cytochrome  c level and diminished growth on YPG, the  pet20-  strain was sensitive to a number of mitochondria-specific drugs, such as: calcium  chloride, which regulates mitochondrial function; oligomycin, an inhibitor of ATP  synthase and oxidative phosphorylation; potassium ferricyanide, an inhibitor of oxidative  phosphorylation; and hydrogen peroxide, a strong oxidant and stress agent that affects  proton/electron balance in the cell (Figure  2B).	gene_phenotype
73239	10	334764	5	NULL	NULL	0	NULL	potassium ferricyanide	Chemical		is an inhibitor of					oxidative phosphorylation	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_282	16491469	In addition to the lower cytochrome  c level and diminished growth on YPG, the  pet20-  strain was sensitive to a number of mitochondria-specific drugs, such as: calcium  chloride, which regulates mitochondrial function; oligomycin, an inhibitor of ATP  synthase and oxidative phosphorylation; potassium ferricyanide, an inhibitor of oxidative  phosphorylation; and hydrogen peroxide, a strong oxidant and stress agent that affects  proton/electron balance in the cell (Figure  2B).	gene_phenotype
73240	11	334764	5	NULL	NULL	0	NULL	pet20- strain	Cell		is sensitive to					hydrogen peroxide	Chemical				NULL		0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_282	16491469	In addition to the lower cytochrome  c level and diminished growth on YPG, the  pet20-  strain was sensitive to a number of mitochondria-specific drugs, such as: calcium  chloride, which regulates mitochondrial function; oligomycin, an inhibitor of ATP  synthase and oxidative phosphorylation; potassium ferricyanide, an inhibitor of oxidative  phosphorylation; and hydrogen peroxide, a strong oxidant and stress agent that affects  proton/electron balance in the cell (Figure  2B).	gene_phenotype
73241	12	334764	5	NULL	NULL	0	NULL	hydrogen peroxide	Chemical		is a type of					mitochondria-specific drug	Chemical				NULL		0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_282	16491469	In addition to the lower cytochrome  c level and diminished growth on YPG, the  pet20-  strain was sensitive to a number of mitochondria-specific drugs, such as: calcium  chloride, which regulates mitochondrial function; oligomycin, an inhibitor of ATP  synthase and oxidative phosphorylation; potassium ferricyanide, an inhibitor of oxidative  phosphorylation; and hydrogen peroxide, a strong oxidant and stress agent that affects  proton/electron balance in the cell (Figure  2B).	gene_phenotype
73242	13	334764	5	NULL	NULL	NULL	NULL	hydrogen peroxide	Chemical		is a type of					strong oxidant	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_yeast_23_2_127_s_282	16491469	In addition to the lower cytochrome  c level and diminished growth on YPG, the  pet20-  strain was sensitive to a number of mitochondria-specific drugs, such as: calcium  chloride, which regulates mitochondrial function; oligomycin, an inhibitor of ATP  synthase and oxidative phosphorylation; potassium ferricyanide, an inhibitor of oxidative  phosphorylation; and hydrogen peroxide, a strong oxidant and stress agent that affects  proton/electron balance in the cell (Figure  2B).	gene_phenotype
73243	14	334764	5	NULL	NULL	0	NULL	hydrogen peroxide	Chemical		is a type of					stress agent	Chemical				NULL		0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_282	16491469	In addition to the lower cytochrome  c level and diminished growth on YPG, the  pet20-  strain was sensitive to a number of mitochondria-specific drugs, such as: calcium  chloride, which regulates mitochondrial function; oligomycin, an inhibitor of ATP  synthase and oxidative phosphorylation; potassium ferricyanide, an inhibitor of oxidative  phosphorylation; and hydrogen peroxide, a strong oxidant and stress agent that affects  proton/electron balance in the cell (Figure  2B).	gene_phenotype
73244	15	334764	5	NULL	NULL	0	NULL	hydrogen peroxide	Chemical		balance					 proton/electron	Chemical				NULL	cell	0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_282	16491469	In addition to the lower cytochrome  c level and diminished growth on YPG, the  pet20-  strain was sensitive to a number of mitochondria-specific drugs, such as: calcium  chloride, which regulates mitochondrial function; oligomycin, an inhibitor of ATP  synthase and oxidative phosphorylation; potassium ferricyanide, an inhibitor of oxidative  phosphorylation; and hydrogen peroxide, a strong oxidant and stress agent that affects  proton/electron balance in the cell (Figure  2B).	gene_phenotype
73245	1	334766	5	NULL	NULL	NULL	NULL	Pet20p	GP		constitutes		may			mitochondrial complex	GP	uncharacterized	non-catalytic subunit		NULL		NULL	NULL	NULL	NULL	gw70_yeast_23_2_127_s_8	16491469	It is also possible that Pet20p may constitute  a non-catalytic subunit of an uncharacterized mitochondrial complex or serve as a  transporter or a coupling factor.	gene_phenotype
73246	2	334766	5	NULL	NULL	0	NULL	Pet20p	GP		serve as		may			transporter	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_8	16491469	It is also possible that Pet20p may constitute  a non-catalytic subunit of an uncharacterized mitochondrial complex or serve as a  transporter or a coupling factor.	gene_phenotype
73247	3	334766	5	NULL	NULL	0	NULL	Pet20p	GP		serve as		may			coupling factor	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_8	16491469	It is also possible that Pet20p may constitute  a non-catalytic subunit of an uncharacterized mitochondrial complex or serve as a  transporter or a coupling factor.	gene_phenotype
73248	1	334792	5	NULL	NULL	0	NULL	Pet20p	GP		is involved in		might be			mitochondrial constituent	CellComponent	correct folding of			NULL		0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_279	16491469	Based on the cytochrome content,  phenotypic analysis, protein localization and mitochondrial potential analysis, we  suggest that Pet20p might be involved in correct folding, positioning or compartmentalization  of some mitochondrial constituent which functions to couple electron chain transport  and/or molecular transport across membranes, but does not intrinsically serve an  enzymatic or structural function.	gene_phenotype
73249	2	334792	5	NULL	NULL	0	NULL	Pet20p	GP		is involved in		might be			mitochondrial constituent	CellComponent	positioning of			NULL		0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_279	16491469	Based on the cytochrome content,  phenotypic analysis, protein localization and mitochondrial potential analysis, we  suggest that Pet20p might be involved in correct folding, positioning or compartmentalization  of some mitochondrial constituent which functions to couple electron chain transport  and/or molecular transport across membranes, but does not intrinsically serve an  enzymatic or structural function.	gene_phenotype
73250	3	334792	5	NULL	NULL	0	NULL	Pet20p	GP		is involved in		might be			mitochondrial constituent	CellComponent	compartmentalization of 			NULL		0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_279	16491469	Based on the cytochrome content,  phenotypic analysis, protein localization and mitochondrial potential analysis, we  suggest that Pet20p might be involved in correct folding, positioning or compartmentalization  of some mitochondrial constituent which functions to couple electron chain transport  and/or molecular transport across membranes, but does not intrinsically serve an  enzymatic or structural function.	gene_phenotype
73251	4	334792	5	NULL	NULL	0	NULL	electron chain 	Chemical	transport of	is coupled to					molecules	AbstractConcept	transport of			NULL	across membranes	0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_279	16491469	Based on the cytochrome content,  phenotypic analysis, protein localization and mitochondrial potential analysis, we  suggest that Pet20p might be involved in correct folding, positioning or compartmentalization  of some mitochondrial constituent which functions to couple electron chain transport  and/or molecular transport across membranes, but does not intrinsically serve an  enzymatic or structural function.	gene_phenotype
73252	5	334792	5	NULL	NULL	0	NULL	mitochondrial constituent	CellComponent		functions in					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_279	16491469	Based on the cytochrome content,  phenotypic analysis, protein localization and mitochondrial potential analysis, we  suggest that Pet20p might be involved in correct folding, positioning or compartmentalization  of some mitochondrial constituent which functions to couple electron chain transport  and/or molecular transport across membranes, but does not intrinsically serve an  enzymatic or structural function.	gene_phenotype
73253	6	334792	5	NULL	NULL	0	NULL	mitochondrial constituent	CellComponent		does not serve					 enzymatic function	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_279	16491469	Based on the cytochrome content,  phenotypic analysis, protein localization and mitochondrial potential analysis, we  suggest that Pet20p might be involved in correct folding, positioning or compartmentalization  of some mitochondrial constituent which functions to couple electron chain transport  and/or molecular transport across membranes, but does not intrinsically serve an  enzymatic or structural function.	gene_phenotype
73263	7	334792	5	NULL	NULL	0	NULL	mitochondrial constituent	CellComponent		does not serve					structural function	Process				NULL		0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_279	16491469	Based on the cytochrome content,  phenotypic analysis, protein localization and mitochondrial potential analysis, we  suggest that Pet20p might be involved in correct folding, positioning or compartmentalization  of some mitochondrial constituent which functions to couple electron chain transport  and/or molecular transport across membranes, but does not intrinsically serve an  enzymatic or structural function.	gene_phenotype
73266	1	334793	5	NULL	NULL	0	NULL	Pet20p	GP	sequence of	is similar to					Ndufa6	GP	sequence of			NULL		0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_281	16491469	The sequence similarities  of Pet20p to the following proteins (Figure  1A) strongly support such suggestion: Ndufa6, NADH dehydrogenase (ubiquinone) 1  subcomplex subunit 6, a mitochondrial inner membrane protein; yeast Cox14p, a mitochondrial  protein that is required for assembly of cytochrome  c oxidase; and ABCA2, a member of the superfamily of ATP-binding cassette (ABC) transporters.	gene_phenotype
73267	2	334793	5	NULL	NULL	0	NULL	Ndufa6	GP		is					NADH dehydrogenase (ubiquinone) 1 subcomplex subunit 6	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_281	16491469	The sequence similarities  of Pet20p to the following proteins (Figure  1A) strongly support such suggestion: Ndufa6, NADH dehydrogenase (ubiquinone) 1  subcomplex subunit 6, a mitochondrial inner membrane protein; yeast Cox14p, a mitochondrial  protein that is required for assembly of cytochrome  c oxidase; and ABCA2, a member of the superfamily of ATP-binding cassette (ABC) transporters.	gene_phenotype
73269	3	334793	5	NULL	NULL	0	NULL	Ndufa6	GP		is a type of					mitochondrial inner membrane protein	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_281	16491469	The sequence similarities  of Pet20p to the following proteins (Figure  1A) strongly support such suggestion: Ndufa6, NADH dehydrogenase (ubiquinone) 1  subcomplex subunit 6, a mitochondrial inner membrane protein; yeast Cox14p, a mitochondrial  protein that is required for assembly of cytochrome  c oxidase; and ABCA2, a member of the superfamily of ATP-binding cassette (ABC) transporters.	gene_phenotype
73270	4	334793	5	NULL	NULL	0	NULL	Pet20p	GP	sequence of	is similar to					Cox14p	GP	sequence of;;yeast			NULL		0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_281	16491469	The sequence similarities  of Pet20p to the following proteins (Figure  1A) strongly support such suggestion: Ndufa6, NADH dehydrogenase (ubiquinone) 1  subcomplex subunit 6, a mitochondrial inner membrane protein; yeast Cox14p, a mitochondrial  protein that is required for assembly of cytochrome  c oxidase; and ABCA2, a member of the superfamily of ATP-binding cassette (ABC) transporters.	gene_phenotype
73272	5	334793	5	NULL	NULL	0	NULL	Cox14p	GP	yeast	is a type of					mitochondrial protein	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_281	16491469	The sequence similarities  of Pet20p to the following proteins (Figure  1A) strongly support such suggestion: Ndufa6, NADH dehydrogenase (ubiquinone) 1  subcomplex subunit 6, a mitochondrial inner membrane protein; yeast Cox14p, a mitochondrial  protein that is required for assembly of cytochrome  c oxidase; and ABCA2, a member of the superfamily of ATP-binding cassette (ABC) transporters.	gene_phenotype
73273	6	334793	5	NULL	NULL	0	NULL	Cox14p	GP	yeast	is required for					cytochrome c oxidase	GP	assembly of			NULL		0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_281	16491469	The sequence similarities  of Pet20p to the following proteins (Figure  1A) strongly support such suggestion: Ndufa6, NADH dehydrogenase (ubiquinone) 1  subcomplex subunit 6, a mitochondrial inner membrane protein; yeast Cox14p, a mitochondrial  protein that is required for assembly of cytochrome  c oxidase; and ABCA2, a member of the superfamily of ATP-binding cassette (ABC) transporters.	gene_phenotype
73275	7	334793	5	NULL	NULL	0	NULL	Pet20p	GP	sequence of	is similar to					ABCA2	GP	sequence of			NULL		0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_281	16491469	The sequence similarities  of Pet20p to the following proteins (Figure  1A) strongly support such suggestion: Ndufa6, NADH dehydrogenase (ubiquinone) 1  subcomplex subunit 6, a mitochondrial inner membrane protein; yeast Cox14p, a mitochondrial  protein that is required for assembly of cytochrome  c oxidase; and ABCA2, a member of the superfamily of ATP-binding cassette (ABC) transporters.	gene_phenotype
73279	8	334793	5	NULL	NULL	0	NULL	ABCA2	GP		is a member of					ABC transporters superfamilty	GP				NULL		0	NULL	NULL	NULL	gw70_yeast_23_2_127_s_281	16491469	The sequence similarities  of Pet20p to the following proteins (Figure  1A) strongly support such suggestion: Ndufa6, NADH dehydrogenase (ubiquinone) 1  subcomplex subunit 6, a mitochondrial inner membrane protein; yeast Cox14p, a mitochondrial  protein that is required for assembly of cytochrome  c oxidase; and ABCA2, a member of the superfamily of ATP-binding cassette (ABC) transporters.	gene_phenotype
73281	9	334793	5	NULL	NULL	NULL	NULL	ABC transporters	GP		is					ATP-binding cassette transporters	GP				NULL		NULL	NULL	NULL	NULL	gw70_yeast_23_2_127_s_281	16491469	The sequence similarities  of Pet20p to the following proteins (Figure  1A) strongly support such suggestion: Ndufa6, NADH dehydrogenase (ubiquinone) 1  subcomplex subunit 6, a mitochondrial inner membrane protein; yeast Cox14p, a mitochondrial  protein that is required for assembly of cytochrome  c oxidase; and ABCA2, a member of the superfamily of ATP-binding cassette (ABC) transporters.	gene_phenotype
73296	1	334801	5	NULL	NULL	0	NULL	LpxP protein	GP	controlled overproduction of	increases					palmitoleoyltransferase activity	Process				NULL	in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_277_16_14186_s_202	11830594	Massive Overproduction of Palmitoleoyltransferase in Cells Expressing lpxP Behind a T7lac Promoter-- The  lpxP gene was cloned into a T7 polymerase expression vector, pET21a+, to confirm that controlled overproduction of the LpxP protein from a non-native promoter results in increased  in vitro palmitoleoyltransferase activity.	gene_phenotype
51560	1	334823	5	NULL	NULL	0	NULL	Cyp 7a	NULL		is	NULL				cholesterol 7alpha-hydroxylase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_35_31441_s_30	12052824	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase (Cyp 7a) ( 14-17), the enzyme catalyzing the first and rate-limiting step of bile acid synthesis ( 18), and activates expression of intestinal bile acid-binding protein ( 11), phospholipid transfer protein ( 19), BSEP ( 20), and dehydroepiandrosterone sulfotransferase ( 21).	transcription
51561	2	334823	5	NULL	NULL	NULL	NULL	FXR			inhibit					Cyp 7a		expression of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_35_31441_s_30	12052824	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase (Cyp 7a) ( 14-17), the enzyme catalyzing the first and rate-limiting step of bile acid synthesis ( 18), and activates expression of intestinal bile acid-binding protein ( 11), phospholipid transfer protein ( 19), BSEP ( 20), and dehydroepiandrosterone sulfotransferase ( 21).	transcription
51562	3	334823	5	NULL	NULL	NULL	NULL	Cyp 7a			catalyzes					bile acid		synthesis of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_35_31441_s_30	12052824	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase (Cyp 7a) ( 14-17), the enzyme catalyzing the first and rate-limiting step of bile acid synthesis ( 18), and activates expression of intestinal bile acid-binding protein ( 11), phospholipid transfer protein ( 19), BSEP ( 20), and dehydroepiandrosterone sulfotransferase ( 21).	transcription
51563	4	334823	5	NULL	NULL	NULL	NULL	FXR			activates					intestinal bile acid-binding protein		expression of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_35_31441_s_30	12052824	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase (Cyp 7a) ( 14-17), the enzyme catalyzing the first and rate-limiting step of bile acid synthesis ( 18), and activates expression of intestinal bile acid-binding protein ( 11), phospholipid transfer protein ( 19), BSEP ( 20), and dehydroepiandrosterone sulfotransferase ( 21).	transcription
51564	5	334823	5	NULL	NULL	NULL	NULL	FXR			activates					phospholipid transfer protein		expression of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_35_31441_s_30	12052824	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase (Cyp 7a) ( 14-17), the enzyme catalyzing the first and rate-limiting step of bile acid synthesis ( 18), and activates expression of intestinal bile acid-binding protein ( 11), phospholipid transfer protein ( 19), BSEP ( 20), and dehydroepiandrosterone sulfotransferase ( 21).	transcription
51565	6	334823	5	NULL	NULL	NULL	NULL	FXR			activates					BSEP		expression of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_35_31441_s_30	12052824	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase (Cyp 7a) ( 14-17), the enzyme catalyzing the first and rate-limiting step of bile acid synthesis ( 18), and activates expression of intestinal bile acid-binding protein ( 11), phospholipid transfer protein ( 19), BSEP ( 20), and dehydroepiandrosterone sulfotransferase ( 21).	transcription
51566	7	334823	5	NULL	NULL	NULL	NULL	FXR			activates					dehydroepiandrosterone sulfotransferase		expression of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_35_31441_s_30	12052824	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase (Cyp 7a) ( 14-17), the enzyme catalyzing the first and rate-limiting step of bile acid synthesis ( 18), and activates expression of intestinal bile acid-binding protein ( 11), phospholipid transfer protein ( 19), BSEP ( 20), and dehydroepiandrosterone sulfotransferase ( 21).	transcription
54318	8	334823	5	NULL	NULL	NULL	NULL	Cyp 7a			is a type of					enzyme					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_35_31441_s_30	12052824	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase (Cyp 7a) ( 14-17), the enzyme catalyzing the first and rate-limiting step of bile acid synthesis ( 18), and activates expression of intestinal bile acid-binding protein ( 11), phospholipid transfer protein ( 19), BSEP ( 20), and dehydroepiandrosterone sulfotransferase ( 21).	transcription
51939	1	334823	6	NULL	NULL	0	NULL	Cyp 7a	NULL		is	NULL				cholesterol 7alpha-hydroxylase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_35_31441_s_30	12052824	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase (Cyp 7a) ( 14-17), the enzyme catalyzing the first and rate-limiting step of bile acid synthesis ( 18), and activates expression of intestinal bile acid-binding protein ( 11), phospholipid transfer protein ( 19), BSEP ( 20), and dehydroepiandrosterone sulfotransferase ( 21).	transcription
51940	2	334823	6	NULL	NULL	0	NULL	Cyp 7a	NULL		is a type of	NULL				enzyme	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_35_31441_s_30	12052824	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase (Cyp 7a) ( 14-17), the enzyme catalyzing the first and rate-limiting step of bile acid synthesis ( 18), and activates expression of intestinal bile acid-binding protein ( 11), phospholipid transfer protein ( 19), BSEP ( 20), and dehydroepiandrosterone sulfotransferase ( 21).	transcription
51941	3	334823	6	NULL	NULL	0	NULL	Cyp 7a	NULL		catalyzes	NULL				bile acid 	NULL	synthesis of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_35_31441_s_30	12052824	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase (Cyp 7a) ( 14-17), the enzyme catalyzing the first and rate-limiting step of bile acid synthesis ( 18), and activates expression of intestinal bile acid-binding protein ( 11), phospholipid transfer protein ( 19), BSEP ( 20), and dehydroepiandrosterone sulfotransferase ( 21).	transcription
51942	4	334823	6	NULL	NULL	0	NULL	FXR	NULL		inhibits	NULL				Cyp 7a	NULL	expression of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_35_31441_s_30	12052824	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase (Cyp 7a) ( 14-17), the enzyme catalyzing the first and rate-limiting step of bile acid synthesis ( 18), and activates expression of intestinal bile acid-binding protein ( 11), phospholipid transfer protein ( 19), BSEP ( 20), and dehydroepiandrosterone sulfotransferase ( 21).	transcription
51943	5	334823	6	NULL	NULL	0	NULL	FXR	NULL		activates	NULL				bile acid-binding protein	NULL	expression of;; intestinal			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_35_31441_s_30	12052824	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase (Cyp 7a) ( 14-17), the enzyme catalyzing the first and rate-limiting step of bile acid synthesis ( 18), and activates expression of intestinal bile acid-binding protein ( 11), phospholipid transfer protein ( 19), BSEP ( 20), and dehydroepiandrosterone sulfotransferase ( 21).	transcription
51944	6	334823	6	NULL	NULL	0	NULL	FXR	NULL		activates	NULL				phospholipid transfer protein	NULL	expression of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_35_31441_s_30	12052824	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase (Cyp 7a) ( 14-17), the enzyme catalyzing the first and rate-limiting step of bile acid synthesis ( 18), and activates expression of intestinal bile acid-binding protein ( 11), phospholipid transfer protein ( 19), BSEP ( 20), and dehydroepiandrosterone sulfotransferase ( 21).	transcription
51945	7	334823	6	NULL	NULL	0	NULL	FXR	NULL		activates	NULL				BSEP	NULL	expression of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_35_31441_s_30	12052824	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase (Cyp 7a) ( 14-17), the enzyme catalyzing the first and rate-limiting step of bile acid synthesis ( 18), and activates expression of intestinal bile acid-binding protein ( 11), phospholipid transfer protein ( 19), BSEP ( 20), and dehydroepiandrosterone sulfotransferase ( 21).	transcription
51946	8	334823	6	NULL	NULL	0	NULL	FXR	NULL		activates	NULL				dehydroepiandrosterone sulfotransferase	NULL	expression of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_35_31441_s_30	12052824	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase (Cyp 7a) ( 14-17), the enzyme catalyzing the first and rate-limiting step of bile acid synthesis ( 18), and activates expression of intestinal bile acid-binding protein ( 11), phospholipid transfer protein ( 19), BSEP ( 20), and dehydroepiandrosterone sulfotransferase ( 21).	transcription
51567	1	334824	5	NULL	NULL	0	NULL	campesterol	NULL		is a substrate of	NULL	hypothesized			DET2	NULL	Arabidopsis			NULL		0	NULL	NULL	NULL	gw60_pnas_94_8_3554_s_70	9108014	Because the hypothesized substrates of  Arabidopsis DET2 in BR biosynthesis is campesterol or its analogs (sitosterol or stigmasterol), which contain a 3beta-hydroxyl,delta5,6 structure, we measured the steroid 5alpha-reductase activity of DET2 toward several radiolabeled steroids with this structure including cholesterol, pregnenolone, and dehydroepiandrosterone.	transcription
51568	2	334824	5	NULL	NULL	0	NULL	statement 1	NULL		plays a role in	NULL				BR	NULL	biosynthesis of			NULL		0	NULL	NULL	NULL	gw60_pnas_94_8_3554_s_70	9108014	Because the hypothesized substrates of  Arabidopsis DET2 in BR biosynthesis is campesterol or its analogs (sitosterol or stigmasterol), which contain a 3beta-hydroxyl,delta5,6 structure, we measured the steroid 5alpha-reductase activity of DET2 toward several radiolabeled steroids with this structure including cholesterol, pregnenolone, and dehydroepiandrosterone.	transcription
51569	3	334824	5	NULL	NULL	0	NULL	sitosterol	NULL		is an analog of	NULL				campesterol	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_94_8_3554_s_70	9108014	Because the hypothesized substrates of  Arabidopsis DET2 in BR biosynthesis is campesterol or its analogs (sitosterol or stigmasterol), which contain a 3beta-hydroxyl,delta5,6 structure, we measured the steroid 5alpha-reductase activity of DET2 toward several radiolabeled steroids with this structure including cholesterol, pregnenolone, and dehydroepiandrosterone.	transcription
51570	4	334824	5	NULL	NULL	0	NULL	stigmasterol	NULL		is an analog of	NULL				campesterol	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_94_8_3554_s_70	9108014	Because the hypothesized substrates of  Arabidopsis DET2 in BR biosynthesis is campesterol or its analogs (sitosterol or stigmasterol), which contain a 3beta-hydroxyl,delta5,6 structure, we measured the steroid 5alpha-reductase activity of DET2 toward several radiolabeled steroids with this structure including cholesterol, pregnenolone, and dehydroepiandrosterone.	transcription
51571	5	334824	5	NULL	NULL	0	NULL	sitosterol	NULL		is a substrate of	NULL	hypothesized			DET2	NULL	Arabidopsis			NULL		0	NULL	NULL	NULL	gw60_pnas_94_8_3554_s_70	9108014	Because the hypothesized substrates of  Arabidopsis DET2 in BR biosynthesis is campesterol or its analogs (sitosterol or stigmasterol), which contain a 3beta-hydroxyl,delta5,6 structure, we measured the steroid 5alpha-reductase activity of DET2 toward several radiolabeled steroids with this structure including cholesterol, pregnenolone, and dehydroepiandrosterone.	transcription
51572	6	334824	5	NULL	NULL	0	NULL	statement 5	NULL		plays a role in	NULL				BR	NULL	biosynthesis of			NULL		0	NULL	NULL	NULL	gw60_pnas_94_8_3554_s_70	9108014	Because the hypothesized substrates of  Arabidopsis DET2 in BR biosynthesis is campesterol or its analogs (sitosterol or stigmasterol), which contain a 3beta-hydroxyl,delta5,6 structure, we measured the steroid 5alpha-reductase activity of DET2 toward several radiolabeled steroids with this structure including cholesterol, pregnenolone, and dehydroepiandrosterone.	transcription
51573	7	334824	5	NULL	NULL	0	NULL	stigmasterol	NULL		is a substrate of	NULL	hypothesized			DET2	NULL	Arabidopsis			NULL		0	NULL	NULL	NULL	gw60_pnas_94_8_3554_s_70	9108014	Because the hypothesized substrates of  Arabidopsis DET2 in BR biosynthesis is campesterol or its analogs (sitosterol or stigmasterol), which contain a 3beta-hydroxyl,delta5,6 structure, we measured the steroid 5alpha-reductase activity of DET2 toward several radiolabeled steroids with this structure including cholesterol, pregnenolone, and dehydroepiandrosterone.	transcription
51574	8	334824	5	NULL	NULL	0	NULL	statement 7	NULL		plays a role in	NULL				BR	NULL	biosynthesis of			NULL		0	NULL	NULL	NULL	gw60_pnas_94_8_3554_s_70	9108014	Because the hypothesized substrates of  Arabidopsis DET2 in BR biosynthesis is campesterol or its analogs (sitosterol or stigmasterol), which contain a 3beta-hydroxyl,delta5,6 structure, we measured the steroid 5alpha-reductase activity of DET2 toward several radiolabeled steroids with this structure including cholesterol, pregnenolone, and dehydroepiandrosterone.	transcription
51947	1	334824	6	NULL	NULL	0	NULL	DET2	NULL	arabidopsis	exhibits	NULL				steroid 5alpha-reductase activity	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_8_3554_s_70	9108014	Because the hypothesized substrates of  Arabidopsis DET2 in BR biosynthesis is campesterol or its analogs (sitosterol or stigmasterol), which contain a 3beta-hydroxyl,delta5,6 structure, we measured the steroid 5alpha-reductase activity of DET2 toward several radiolabeled steroids with this structure including cholesterol, pregnenolone, and dehydroepiandrosterone.	transcription
51948	2	334824	6	NULL	NULL	0	NULL	campesterol	NULL		contains	NULL				3beta-hydroxyl,delta5,6 structure	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_8_3554_s_70	9108014	Because the hypothesized substrates of  Arabidopsis DET2 in BR biosynthesis is campesterol or its analogs (sitosterol or stigmasterol), which contain a 3beta-hydroxyl,delta5,6 structure, we measured the steroid 5alpha-reductase activity of DET2 toward several radiolabeled steroids with this structure including cholesterol, pregnenolone, and dehydroepiandrosterone.	transcription
51949	3	334824	6	NULL	NULL	0	NULL	sitosterol	NULL		contains	NULL				3beta-hydroxyl,delta5,6 structure	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_94_8_3554_s_70	9108014	Because the hypothesized substrates of  Arabidopsis DET2 in BR biosynthesis is campesterol or its analogs (sitosterol or stigmasterol), which contain a 3beta-hydroxyl,delta5,6 structure, we measured the steroid 5alpha-reductase activity of DET2 toward several radiolabeled steroids with this structure including cholesterol, pregnenolone, and dehydroepiandrosterone.	transcription
51950	4	334824	6	NULL	NULL	0	NULL	stigmasterol	NULL		contains	NULL				3beta-hydroxyl,delta5,6 structure	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_94_8_3554_s_70	9108014	Because the hypothesized substrates of  Arabidopsis DET2 in BR biosynthesis is campesterol or its analogs (sitosterol or stigmasterol), which contain a 3beta-hydroxyl,delta5,6 structure, we measured the steroid 5alpha-reductase activity of DET2 toward several radiolabeled steroids with this structure including cholesterol, pregnenolone, and dehydroepiandrosterone.	transcription
51575	1	334825	5	NULL	NULL	0	NULL	Cyp 7a1	NULL		is	NULL				cholesterol 7alpha-hydroxylase	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10214_s_20	12525500	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase ( Cyp 7a1) ( ), sterol 12alpha-hydroxylase ( ), the Na+/taurocholate co-transporting polypeptide ( ) and apolipoprotein A-I ( ), and activates expression of intestinal bile acid-binding protein ( I-BABP) ( ), phospholipid transfer protein ( ), bile salt export pump ( BSEP) ( ,  ), dehydroepiandrosterone sulfotransferase ( ), and apolipoprotein C-II ( ).	transcription
51576	2	334825	5	NULL	NULL	0	NULL	FXR	NULL		inhibit	NULL				Cyp 7a1	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10214_s_20	12525500	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase ( Cyp 7a1) ( ), sterol 12alpha-hydroxylase ( ), the Na+/taurocholate co-transporting polypeptide ( ) and apolipoprotein A-I ( ), and activates expression of intestinal bile acid-binding protein ( I-BABP) ( ), phospholipid transfer protein ( ), bile salt export pump ( BSEP) ( ,  ), dehydroepiandrosterone sulfotransferase ( ), and apolipoprotein C-II ( ).	transcription
51577	3	334825	5	NULL	NULL	0	NULL	FXR	NULL		inhibit	NULL				sterol 12alpha-hydroxylase	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10214_s_20	12525500	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase ( Cyp 7a1) ( ), sterol 12alpha-hydroxylase ( ), the Na+/taurocholate co-transporting polypeptide ( ) and apolipoprotein A-I ( ), and activates expression of intestinal bile acid-binding protein ( I-BABP) ( ), phospholipid transfer protein ( ), bile salt export pump ( BSEP) ( ,  ), dehydroepiandrosterone sulfotransferase ( ), and apolipoprotein C-II ( ).	transcription
51578	4	334825	5	NULL	NULL	0	NULL	FXR	NULL		inhibit	NULL				Na+/taurocholate co-transporting polypeptide	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10214_s_20	12525500	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase ( Cyp 7a1) ( ), sterol 12alpha-hydroxylase ( ), the Na+/taurocholate co-transporting polypeptide ( ) and apolipoprotein A-I ( ), and activates expression of intestinal bile acid-binding protein ( I-BABP) ( ), phospholipid transfer protein ( ), bile salt export pump ( BSEP) ( ,  ), dehydroepiandrosterone sulfotransferase ( ), and apolipoprotein C-II ( ).	transcription
51579	5	334825	5	NULL	NULL	0	NULL	FXR	NULL		inhibit	NULL				apolipoprotein A-I	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10214_s_20	12525500	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase ( Cyp 7a1) ( ), sterol 12alpha-hydroxylase ( ), the Na+/taurocholate co-transporting polypeptide ( ) and apolipoprotein A-I ( ), and activates expression of intestinal bile acid-binding protein ( I-BABP) ( ), phospholipid transfer protein ( ), bile salt export pump ( BSEP) ( ,  ), dehydroepiandrosterone sulfotransferase ( ), and apolipoprotein C-II ( ).	transcription
51580	6	334825	5	NULL	NULL	0	NULL	I-BABP	NULL		is	NULL				intestinal bile acid-binding protein	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10214_s_20	12525500	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase ( Cyp 7a1) ( ), sterol 12alpha-hydroxylase ( ), the Na+/taurocholate co-transporting polypeptide ( ) and apolipoprotein A-I ( ), and activates expression of intestinal bile acid-binding protein ( I-BABP) ( ), phospholipid transfer protein ( ), bile salt export pump ( BSEP) ( ,  ), dehydroepiandrosterone sulfotransferase ( ), and apolipoprotein C-II ( ).	transcription
51581	7	334825	5	NULL	NULL	0	NULL	FXR	NULL		activates	NULL				I-BABP	NULL	expression of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_12_10214_s_20	12525500	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase ( Cyp 7a1) ( ), sterol 12alpha-hydroxylase ( ), the Na+/taurocholate co-transporting polypeptide ( ) and apolipoprotein A-I ( ), and activates expression of intestinal bile acid-binding protein ( I-BABP) ( ), phospholipid transfer protein ( ), bile salt export pump ( BSEP) ( ,  ), dehydroepiandrosterone sulfotransferase ( ), and apolipoprotein C-II ( ).	transcription
51582	8	334825	5	NULL	NULL	0	NULL	FXR	NULL		activates	NULL				phospholipid transfer protein	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10214_s_20	12525500	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase ( Cyp 7a1) ( ), sterol 12alpha-hydroxylase ( ), the Na+/taurocholate co-transporting polypeptide ( ) and apolipoprotein A-I ( ), and activates expression of intestinal bile acid-binding protein ( I-BABP) ( ), phospholipid transfer protein ( ), bile salt export pump ( BSEP) ( ,  ), dehydroepiandrosterone sulfotransferase ( ), and apolipoprotein C-II ( ).	transcription
51583	9	334825	5	NULL	NULL	0	NULL	BSEP	NULL		is	NULL				bile salt export pump	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10214_s_20	12525500	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase ( Cyp 7a1) ( ), sterol 12alpha-hydroxylase ( ), the Na+/taurocholate co-transporting polypeptide ( ) and apolipoprotein A-I ( ), and activates expression of intestinal bile acid-binding protein ( I-BABP) ( ), phospholipid transfer protein ( ), bile salt export pump ( BSEP) ( ,  ), dehydroepiandrosterone sulfotransferase ( ), and apolipoprotein C-II ( ).	transcription
51584	10	334825	5	NULL	NULL	0	NULL	FXR	NULL		activates	NULL				BSEP	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10214_s_20	12525500	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase ( Cyp 7a1) ( ), sterol 12alpha-hydroxylase ( ), the Na+/taurocholate co-transporting polypeptide ( ) and apolipoprotein A-I ( ), and activates expression of intestinal bile acid-binding protein ( I-BABP) ( ), phospholipid transfer protein ( ), bile salt export pump ( BSEP) ( ,  ), dehydroepiandrosterone sulfotransferase ( ), and apolipoprotein C-II ( ).	transcription
51585	11	334825	5	NULL	NULL	0	NULL	FXR	NULL		activates	NULL				dehydroepiandrosterone sulfotransferase	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10214_s_20	12525500	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase ( Cyp 7a1) ( ), sterol 12alpha-hydroxylase ( ), the Na+/taurocholate co-transporting polypeptide ( ) and apolipoprotein A-I ( ), and activates expression of intestinal bile acid-binding protein ( I-BABP) ( ), phospholipid transfer protein ( ), bile salt export pump ( BSEP) ( ,  ), dehydroepiandrosterone sulfotransferase ( ), and apolipoprotein C-II ( ).	transcription
51586	12	334825	5	NULL	NULL	0	NULL	FXR	NULL		activates	NULL				apolipoprotein C-II	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10214_s_20	12525500	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase ( Cyp 7a1) ( ), sterol 12alpha-hydroxylase ( ), the Na+/taurocholate co-transporting polypeptide ( ) and apolipoprotein A-I ( ), and activates expression of intestinal bile acid-binding protein ( I-BABP) ( ), phospholipid transfer protein ( ), bile salt export pump ( BSEP) ( ,  ), dehydroepiandrosterone sulfotransferase ( ), and apolipoprotein C-II ( ).	transcription
51951	1	334825	6	NULL	NULL	0	NULL	FXR	NULL		inhibits	NULL				Cyp 7a1	NULL	expression of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10214_s_20	12525500	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase ( Cyp 7a1) ( ), sterol 12alpha-hydroxylase ( ), the Na+/taurocholate co-transporting polypeptide ( ) and apolipoprotein A-I ( ), and activates expression of intestinal bile acid-binding protein ( I-BABP) ( ), phospholipid transfer protein ( ), bile salt export pump ( BSEP) ( ,  ), dehydroepiandrosterone sulfotransferase ( ), and apolipoprotein C-II ( ).	transcription
51952	2	334825	6	NULL	NULL	0	NULL	Cyp 7a	NULL		is	NULL				cholesterol 7alpha-hydroxylase	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10214_s_20	12525500	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase ( Cyp 7a1) ( ), sterol 12alpha-hydroxylase ( ), the Na+/taurocholate co-transporting polypeptide ( ) and apolipoprotein A-I ( ), and activates expression of intestinal bile acid-binding protein ( I-BABP) ( ), phospholipid transfer protein ( ), bile salt export pump ( BSEP) ( ,  ), dehydroepiandrosterone sulfotransferase ( ), and apolipoprotein C-II ( ).	transcription
51953	3	334825	6	NULL	NULL	0	NULL	FXR	NULL		inhibits	NULL				sterol 12alpha-hydroxylase	NULL	expression of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10214_s_20	12525500	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase ( Cyp 7a1) ( ), sterol 12alpha-hydroxylase ( ), the Na+/taurocholate co-transporting polypeptide ( ) and apolipoprotein A-I ( ), and activates expression of intestinal bile acid-binding protein ( I-BABP) ( ), phospholipid transfer protein ( ), bile salt export pump ( BSEP) ( ,  ), dehydroepiandrosterone sulfotransferase ( ), and apolipoprotein C-II ( ).	transcription
51954	4	334825	6	NULL	NULL	0	NULL	FXR	NULL		inhibits	NULL				Na+/taurocholate co-transporting polypeptide	NULL	expression of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10214_s_20	12525500	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase ( Cyp 7a1) ( ), sterol 12alpha-hydroxylase ( ), the Na+/taurocholate co-transporting polypeptide ( ) and apolipoprotein A-I ( ), and activates expression of intestinal bile acid-binding protein ( I-BABP) ( ), phospholipid transfer protein ( ), bile salt export pump ( BSEP) ( ,  ), dehydroepiandrosterone sulfotransferase ( ), and apolipoprotein C-II ( ).	transcription
51955	5	334825	6	NULL	NULL	0	NULL	FXR	NULL		inhibits	NULL				apolipoprotein A-I	NULL	expression of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10214_s_20	12525500	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase ( Cyp 7a1) ( ), sterol 12alpha-hydroxylase ( ), the Na+/taurocholate co-transporting polypeptide ( ) and apolipoprotein A-I ( ), and activates expression of intestinal bile acid-binding protein ( I-BABP) ( ), phospholipid transfer protein ( ), bile salt export pump ( BSEP) ( ,  ), dehydroepiandrosterone sulfotransferase ( ), and apolipoprotein C-II ( ).	transcription
51956	6	334825	6	NULL	NULL	0	NULL	I-BABP	NULL		is	NULL				intestinal bile acid-binding protein	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10214_s_20	12525500	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase ( Cyp 7a1) ( ), sterol 12alpha-hydroxylase ( ), the Na+/taurocholate co-transporting polypeptide ( ) and apolipoprotein A-I ( ), and activates expression of intestinal bile acid-binding protein ( I-BABP) ( ), phospholipid transfer protein ( ), bile salt export pump ( BSEP) ( ,  ), dehydroepiandrosterone sulfotransferase ( ), and apolipoprotein C-II ( ).	transcription
51957	7	334825	6	NULL	NULL	0	NULL	FXR	NULL		activates	NULL				I-BABP	NULL	expression of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10214_s_20	12525500	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase ( Cyp 7a1) ( ), sterol 12alpha-hydroxylase ( ), the Na+/taurocholate co-transporting polypeptide ( ) and apolipoprotein A-I ( ), and activates expression of intestinal bile acid-binding protein ( I-BABP) ( ), phospholipid transfer protein ( ), bile salt export pump ( BSEP) ( ,  ), dehydroepiandrosterone sulfotransferase ( ), and apolipoprotein C-II ( ).	transcription
51958	8	334825	6	NULL	NULL	0	NULL	FXR	NULL		activates	NULL				phospholipid transfer protein	NULL	expression of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10214_s_20	12525500	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase ( Cyp 7a1) ( ), sterol 12alpha-hydroxylase ( ), the Na+/taurocholate co-transporting polypeptide ( ) and apolipoprotein A-I ( ), and activates expression of intestinal bile acid-binding protein ( I-BABP) ( ), phospholipid transfer protein ( ), bile salt export pump ( BSEP) ( ,  ), dehydroepiandrosterone sulfotransferase ( ), and apolipoprotein C-II ( ).	transcription
51959	9	334825	6	NULL	NULL	0	NULL	BSEP	NULL		is	NULL				bile salt export pump	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10214_s_20	12525500	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase ( Cyp 7a1) ( ), sterol 12alpha-hydroxylase ( ), the Na+/taurocholate co-transporting polypeptide ( ) and apolipoprotein A-I ( ), and activates expression of intestinal bile acid-binding protein ( I-BABP) ( ), phospholipid transfer protein ( ), bile salt export pump ( BSEP) ( ,  ), dehydroepiandrosterone sulfotransferase ( ), and apolipoprotein C-II ( ).	transcription
51960	10	334825	6	NULL	NULL	0	NULL	FXR	NULL		activates	NULL				BSEP	NULL	expression of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10214_s_20	12525500	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase ( Cyp 7a1) ( ), sterol 12alpha-hydroxylase ( ), the Na+/taurocholate co-transporting polypeptide ( ) and apolipoprotein A-I ( ), and activates expression of intestinal bile acid-binding protein ( I-BABP) ( ), phospholipid transfer protein ( ), bile salt export pump ( BSEP) ( ,  ), dehydroepiandrosterone sulfotransferase ( ), and apolipoprotein C-II ( ).	transcription
51961	11	334825	6	NULL	NULL	0	NULL	FXR	NULL		activates	NULL				dehydroepiandrosterone sulfotransferase	NULL	expression of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10214_s_20	12525500	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase ( Cyp 7a1) ( ), sterol 12alpha-hydroxylase ( ), the Na+/taurocholate co-transporting polypeptide ( ) and apolipoprotein A-I ( ), and activates expression of intestinal bile acid-binding protein ( I-BABP) ( ), phospholipid transfer protein ( ), bile salt export pump ( BSEP) ( ,  ), dehydroepiandrosterone sulfotransferase ( ), and apolipoprotein C-II ( ).	transcription
51962	12	334825	6	NULL	NULL	0	NULL	FXR	NULL		activates	NULL				apolipoprotein C-II	NULL	expression of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10214_s_20	12525500	It has been shown that FXR inhibits expression of cholesterol 7alpha-hydroxylase ( Cyp 7a1) ( ), sterol 12alpha-hydroxylase ( ), the Na+/taurocholate co-transporting polypeptide ( ) and apolipoprotein A-I ( ), and activates expression of intestinal bile acid-binding protein ( I-BABP) ( ), phospholipid transfer protein ( ), bile salt export pump ( BSEP) ( ,  ), dehydroepiandrosterone sulfotransferase ( ), and apolipoprotein C-II ( ).	transcription
51587	1	334826	5	NULL	NULL	0	NULL	SF1	NULL		is a type of	NULL				steroidogenic factor	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_279_2_271_s_287	15733658	In addition, the adult ovary gene set included all relevant steroidogenic regulators  and enzymes that are expressed in luteal cells and adult stroma (including steroidogenic  factor  SF1 (H3053B11, confirmatory data in  Fig. 4), which regulates transcription of all cytochrome  P450s; P450ssc/Cyp11A1 (H3094D01), catalyzing the conversion of cholesterol to pregnenolone;  steroidogenic acute regulatory protein StAR (H3097G04), which regulates accessibility  of cholesterol to P450ssc; P450c17/Cyp17 (H3018A11), a theca cell marker that catalyzes  the formation of dehydroepiandrosterone (DHEA) and is upregulated by Gdf9 in preantral  follicles (  Vitt et al., 2000); and two clones (H3059B01, H3070C08) for placental 3- -hydroxysteroid dehydrogenase  Hsd3b1 (see OMIM109715)).	transcription
51588	2	334826	5	NULL	NULL	0	NULL	SF1	NULL		regulates	NULL				cytochrome P450s	NULL	transcription of			NULL		0	NULL	NULL	NULL	gw70_devbiol_279_2_271_s_287	15733658	In addition, the adult ovary gene set included all relevant steroidogenic regulators  and enzymes that are expressed in luteal cells and adult stroma (including steroidogenic  factor  SF1 (H3053B11, confirmatory data in  Fig. 4), which regulates transcription of all cytochrome  P450s; P450ssc/Cyp11A1 (H3094D01), catalyzing the conversion of cholesterol to pregnenolone;  steroidogenic acute regulatory protein StAR (H3097G04), which regulates accessibility  of cholesterol to P450ssc; P450c17/Cyp17 (H3018A11), a theca cell marker that catalyzes  the formation of dehydroepiandrosterone (DHEA) and is upregulated by Gdf9 in preantral  follicles (  Vitt et al., 2000); and two clones (H3059B01, H3070C08) for placental 3- -hydroxysteroid dehydrogenase  Hsd3b1 (see OMIM109715)).	transcription
51590	3	334826	5	NULL	NULL	0	NULL	cholesterol	NULL		is converted to	NULL				pregnenolone	NULL				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_279_2_271_s_287	15733658	In addition, the adult ovary gene set included all relevant steroidogenic regulators  and enzymes that are expressed in luteal cells and adult stroma (including steroidogenic  factor  SF1 (H3053B11, confirmatory data in  Fig. 4), which regulates transcription of all cytochrome  P450s; P450ssc/Cyp11A1 (H3094D01), catalyzing the conversion of cholesterol to pregnenolone;  steroidogenic acute regulatory protein StAR (H3097G04), which regulates accessibility  of cholesterol to P450ssc; P450c17/Cyp17 (H3018A11), a theca cell marker that catalyzes  the formation of dehydroepiandrosterone (DHEA) and is upregulated by Gdf9 in preantral  follicles (  Vitt et al., 2000); and two clones (H3059B01, H3070C08) for placental 3- -hydroxysteroid dehydrogenase  Hsd3b1 (see OMIM109715)).	transcription
51591	4	334826	5	NULL	NULL	0	NULL	P450ssc/Cyp11A1	NULL		catalyzes	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_279_2_271_s_287	15733658	In addition, the adult ovary gene set included all relevant steroidogenic regulators  and enzymes that are expressed in luteal cells and adult stroma (including steroidogenic  factor  SF1 (H3053B11, confirmatory data in  Fig. 4), which regulates transcription of all cytochrome  P450s; P450ssc/Cyp11A1 (H3094D01), catalyzing the conversion of cholesterol to pregnenolone;  steroidogenic acute regulatory protein StAR (H3097G04), which regulates accessibility  of cholesterol to P450ssc; P450c17/Cyp17 (H3018A11), a theca cell marker that catalyzes  the formation of dehydroepiandrosterone (DHEA) and is upregulated by Gdf9 in preantral  follicles (  Vitt et al., 2000); and two clones (H3059B01, H3070C08) for placental 3- -hydroxysteroid dehydrogenase  Hsd3b1 (see OMIM109715)).	transcription
51592	5	334826	5	NULL	NULL	0	NULL	StAR	NULL		is a type of	NULL				steroidogenic acute regulatory protein	NULL				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_279_2_271_s_287	15733658	In addition, the adult ovary gene set included all relevant steroidogenic regulators  and enzymes that are expressed in luteal cells and adult stroma (including steroidogenic  factor  SF1 (H3053B11, confirmatory data in  Fig. 4), which regulates transcription of all cytochrome  P450s; P450ssc/Cyp11A1 (H3094D01), catalyzing the conversion of cholesterol to pregnenolone;  steroidogenic acute regulatory protein StAR (H3097G04), which regulates accessibility  of cholesterol to P450ssc; P450c17/Cyp17 (H3018A11), a theca cell marker that catalyzes  the formation of dehydroepiandrosterone (DHEA) and is upregulated by Gdf9 in preantral  follicles (  Vitt et al., 2000); and two clones (H3059B01, H3070C08) for placental 3- -hydroxysteroid dehydrogenase  Hsd3b1 (see OMIM109715)).	transcription
51593	6	334826	5	NULL	NULL	0	NULL	cholesterol	NULL		is accessible to	NULL				P450ssc	NULL				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_279_2_271_s_287	15733658	In addition, the adult ovary gene set included all relevant steroidogenic regulators  and enzymes that are expressed in luteal cells and adult stroma (including steroidogenic  factor  SF1 (H3053B11, confirmatory data in  Fig. 4), which regulates transcription of all cytochrome  P450s; P450ssc/Cyp11A1 (H3094D01), catalyzing the conversion of cholesterol to pregnenolone;  steroidogenic acute regulatory protein StAR (H3097G04), which regulates accessibility  of cholesterol to P450ssc; P450c17/Cyp17 (H3018A11), a theca cell marker that catalyzes  the formation of dehydroepiandrosterone (DHEA) and is upregulated by Gdf9 in preantral  follicles (  Vitt et al., 2000); and two clones (H3059B01, H3070C08) for placental 3- -hydroxysteroid dehydrogenase  Hsd3b1 (see OMIM109715)).	transcription
51594	7	334826	5	NULL	NULL	0	NULL	StAR	NULL		regulates	NULL				statement 6	NULL				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_279_2_271_s_287	15733658	In addition, the adult ovary gene set included all relevant steroidogenic regulators  and enzymes that are expressed in luteal cells and adult stroma (including steroidogenic  factor  SF1 (H3053B11, confirmatory data in  Fig. 4), which regulates transcription of all cytochrome  P450s; P450ssc/Cyp11A1 (H3094D01), catalyzing the conversion of cholesterol to pregnenolone;  steroidogenic acute regulatory protein StAR (H3097G04), which regulates accessibility  of cholesterol to P450ssc; P450c17/Cyp17 (H3018A11), a theca cell marker that catalyzes  the formation of dehydroepiandrosterone (DHEA) and is upregulated by Gdf9 in preantral  follicles (  Vitt et al., 2000); and two clones (H3059B01, H3070C08) for placental 3- -hydroxysteroid dehydrogenase  Hsd3b1 (see OMIM109715)).	transcription
51596	8	334826	5	NULL	NULL	0	NULL	P450c17/Cyp17	NULL		is a type of	NULL				theca cell marker	NULL				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_279_2_271_s_287	15733658	In addition, the adult ovary gene set included all relevant steroidogenic regulators  and enzymes that are expressed in luteal cells and adult stroma (including steroidogenic  factor  SF1 (H3053B11, confirmatory data in  Fig. 4), which regulates transcription of all cytochrome  P450s; P450ssc/Cyp11A1 (H3094D01), catalyzing the conversion of cholesterol to pregnenolone;  steroidogenic acute regulatory protein StAR (H3097G04), which regulates accessibility  of cholesterol to P450ssc; P450c17/Cyp17 (H3018A11), a theca cell marker that catalyzes  the formation of dehydroepiandrosterone (DHEA) and is upregulated by Gdf9 in preantral  follicles (  Vitt et al., 2000); and two clones (H3059B01, H3070C08) for placental 3- -hydroxysteroid dehydrogenase  Hsd3b1 (see OMIM109715)).	transcription
51597	9	334826	5	NULL	NULL	0	NULL	P450c17/Cyp17	NULL		catalyzes	NULL				DHEA	NULL	formation of			NULL		NULL	NULL	NULL	NULL	gw70_devbiol_279_2_271_s_287	15733658	In addition, the adult ovary gene set included all relevant steroidogenic regulators  and enzymes that are expressed in luteal cells and adult stroma (including steroidogenic  factor  SF1 (H3053B11, confirmatory data in  Fig. 4), which regulates transcription of all cytochrome  P450s; P450ssc/Cyp11A1 (H3094D01), catalyzing the conversion of cholesterol to pregnenolone;  steroidogenic acute regulatory protein StAR (H3097G04), which regulates accessibility  of cholesterol to P450ssc; P450c17/Cyp17 (H3018A11), a theca cell marker that catalyzes  the formation of dehydroepiandrosterone (DHEA) and is upregulated by Gdf9 in preantral  follicles (  Vitt et al., 2000); and two clones (H3059B01, H3070C08) for placental 3- -hydroxysteroid dehydrogenase  Hsd3b1 (see OMIM109715)).	transcription
51598	10	334826	5	NULL	NULL	0	NULL	DHEA	NULL		is	NULL				dehydroepiandrosterone	NULL				NULL		NULL	NULL	NULL	NULL	gw70_devbiol_279_2_271_s_287	15733658	In addition, the adult ovary gene set included all relevant steroidogenic regulators  and enzymes that are expressed in luteal cells and adult stroma (including steroidogenic  factor  SF1 (H3053B11, confirmatory data in  Fig. 4), which regulates transcription of all cytochrome  P450s; P450ssc/Cyp11A1 (H3094D01), catalyzing the conversion of cholesterol to pregnenolone;  steroidogenic acute regulatory protein StAR (H3097G04), which regulates accessibility  of cholesterol to P450ssc; P450c17/Cyp17 (H3018A11), a theca cell marker that catalyzes  the formation of dehydroepiandrosterone (DHEA) and is upregulated by Gdf9 in preantral  follicles (  Vitt et al., 2000); and two clones (H3059B01, H3070C08) for placental 3- -hydroxysteroid dehydrogenase  Hsd3b1 (see OMIM109715)).	transcription
51599	11	334826	5	NULL	NULL	0	NULL	P450c17/Cyp17	NULL		is upregulated by	NULL				Gdf9	NULL				NULL	preantral follicles	NULL	NULL	NULL	NULL	gw70_devbiol_279_2_271_s_287	15733658	In addition, the adult ovary gene set included all relevant steroidogenic regulators  and enzymes that are expressed in luteal cells and adult stroma (including steroidogenic  factor  SF1 (H3053B11, confirmatory data in  Fig. 4), which regulates transcription of all cytochrome  P450s; P450ssc/Cyp11A1 (H3094D01), catalyzing the conversion of cholesterol to pregnenolone;  steroidogenic acute regulatory protein StAR (H3097G04), which regulates accessibility  of cholesterol to P450ssc; P450c17/Cyp17 (H3018A11), a theca cell marker that catalyzes  the formation of dehydroepiandrosterone (DHEA) and is upregulated by Gdf9 in preantral  follicles (  Vitt et al., 2000); and two clones (H3059B01, H3070C08) for placental 3- -hydroxysteroid dehydrogenase  Hsd3b1 (see OMIM109715)).	transcription
52906	1	334826	6	NULL	NULL	0	NULL	SF1	NULL		is expressed in	NULL				luteal cells	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_279_2_271_s_287	15733658	In addition, the adult ovary gene set included all relevant steroidogenic regulators  and enzymes that are expressed in luteal cells and adult stroma (including steroidogenic  factor  SF1 (H3053B11, confirmatory data in  Fig. 4), which regulates transcription of all cytochrome  P450s; P450ssc/Cyp11A1 (H3094D01), catalyzing the conversion of cholesterol to pregnenolone;  steroidogenic acute regulatory protein StAR (H3097G04), which regulates accessibility  of cholesterol to P450ssc; P450c17/Cyp17 (H3018A11), a theca cell marker that catalyzes  the formation of dehydroepiandrosterone (DHEA) and is upregulated by Gdf9 in preantral  follicles (  Vitt et al., 2000); and two clones (H3059B01, H3070C08) for placental 3- -hydroxysteroid dehydrogenase  Hsd3b1 (see OMIM109715)).	transcription
52907	2	334826	6	NULL	NULL	0	NULL	SF1	NULL		is expressed in	NULL				stroma	NULL	adult			NULL		0	NULL	NULL	NULL	gw70_devbiol_279_2_271_s_287	15733658	In addition, the adult ovary gene set included all relevant steroidogenic regulators  and enzymes that are expressed in luteal cells and adult stroma (including steroidogenic  factor  SF1 (H3053B11, confirmatory data in  Fig. 4), which regulates transcription of all cytochrome  P450s; P450ssc/Cyp11A1 (H3094D01), catalyzing the conversion of cholesterol to pregnenolone;  steroidogenic acute regulatory protein StAR (H3097G04), which regulates accessibility  of cholesterol to P450ssc; P450c17/Cyp17 (H3018A11), a theca cell marker that catalyzes  the formation of dehydroepiandrosterone (DHEA) and is upregulated by Gdf9 in preantral  follicles (  Vitt et al., 2000); and two clones (H3059B01, H3070C08) for placental 3- -hydroxysteroid dehydrogenase  Hsd3b1 (see OMIM109715)).	transcription
52908	3	334826	6	NULL	NULL	0	NULL	SF1	NULL		is	NULL				steroidogenic factor 1	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_279_2_271_s_287	15733658	In addition, the adult ovary gene set included all relevant steroidogenic regulators  and enzymes that are expressed in luteal cells and adult stroma (including steroidogenic  factor  SF1 (H3053B11, confirmatory data in  Fig. 4), which regulates transcription of all cytochrome  P450s; P450ssc/Cyp11A1 (H3094D01), catalyzing the conversion of cholesterol to pregnenolone;  steroidogenic acute regulatory protein StAR (H3097G04), which regulates accessibility  of cholesterol to P450ssc; P450c17/Cyp17 (H3018A11), a theca cell marker that catalyzes  the formation of dehydroepiandrosterone (DHEA) and is upregulated by Gdf9 in preantral  follicles (  Vitt et al., 2000); and two clones (H3059B01, H3070C08) for placental 3- -hydroxysteroid dehydrogenase  Hsd3b1 (see OMIM109715)).	transcription
52909	4	334826	6	NULL	NULL	0	NULL	SF1	NULL		regulates	NULL				cytochrome P450	NULL	transcription of 			NULL		0	NULL	NULL	NULL	gw70_devbiol_279_2_271_s_287	15733658	In addition, the adult ovary gene set included all relevant steroidogenic regulators  and enzymes that are expressed in luteal cells and adult stroma (including steroidogenic  factor  SF1 (H3053B11, confirmatory data in  Fig. 4), which regulates transcription of all cytochrome  P450s; P450ssc/Cyp11A1 (H3094D01), catalyzing the conversion of cholesterol to pregnenolone;  steroidogenic acute regulatory protein StAR (H3097G04), which regulates accessibility  of cholesterol to P450ssc; P450c17/Cyp17 (H3018A11), a theca cell marker that catalyzes  the formation of dehydroepiandrosterone (DHEA) and is upregulated by Gdf9 in preantral  follicles (  Vitt et al., 2000); and two clones (H3059B01, H3070C08) for placental 3- -hydroxysteroid dehydrogenase  Hsd3b1 (see OMIM109715)).	transcription
52910	5	334826	6	NULL	NULL	0	NULL	SF1	NULL		is	NULL				H3053B11	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_279_2_271_s_287	15733658	In addition, the adult ovary gene set included all relevant steroidogenic regulators  and enzymes that are expressed in luteal cells and adult stroma (including steroidogenic  factor  SF1 (H3053B11, confirmatory data in  Fig. 4), which regulates transcription of all cytochrome  P450s; P450ssc/Cyp11A1 (H3094D01), catalyzing the conversion of cholesterol to pregnenolone;  steroidogenic acute regulatory protein StAR (H3097G04), which regulates accessibility  of cholesterol to P450ssc; P450c17/Cyp17 (H3018A11), a theca cell marker that catalyzes  the formation of dehydroepiandrosterone (DHEA) and is upregulated by Gdf9 in preantral  follicles (  Vitt et al., 2000); and two clones (H3059B01, H3070C08) for placental 3- -hydroxysteroid dehydrogenase  Hsd3b1 (see OMIM109715)).	transcription
52911	6	334826	6	NULL	NULL	0	NULL	cholesterol	NULL		is converted to	NULL				pregnenolone	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_279_2_271_s_287	15733658	In addition, the adult ovary gene set included all relevant steroidogenic regulators  and enzymes that are expressed in luteal cells and adult stroma (including steroidogenic  factor  SF1 (H3053B11, confirmatory data in  Fig. 4), which regulates transcription of all cytochrome  P450s; P450ssc/Cyp11A1 (H3094D01), catalyzing the conversion of cholesterol to pregnenolone;  steroidogenic acute regulatory protein StAR (H3097G04), which regulates accessibility  of cholesterol to P450ssc; P450c17/Cyp17 (H3018A11), a theca cell marker that catalyzes  the formation of dehydroepiandrosterone (DHEA) and is upregulated by Gdf9 in preantral  follicles (  Vitt et al., 2000); and two clones (H3059B01, H3070C08) for placental 3- -hydroxysteroid dehydrogenase  Hsd3b1 (see OMIM109715)).	transcription
52912	7	334826	6	NULL	NULL	0	NULL	P450ssc	NULL		catalyzes	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_279_2_271_s_287	15733658	In addition, the adult ovary gene set included all relevant steroidogenic regulators  and enzymes that are expressed in luteal cells and adult stroma (including steroidogenic  factor  SF1 (H3053B11, confirmatory data in  Fig. 4), which regulates transcription of all cytochrome  P450s; P450ssc/Cyp11A1 (H3094D01), catalyzing the conversion of cholesterol to pregnenolone;  steroidogenic acute regulatory protein StAR (H3097G04), which regulates accessibility  of cholesterol to P450ssc; P450c17/Cyp17 (H3018A11), a theca cell marker that catalyzes  the formation of dehydroepiandrosterone (DHEA) and is upregulated by Gdf9 in preantral  follicles (  Vitt et al., 2000); and two clones (H3059B01, H3070C08) for placental 3- -hydroxysteroid dehydrogenase  Hsd3b1 (see OMIM109715)).	transcription
52913	8	334826	6	NULL	NULL	0	NULL	P450ssc	NULL		is	NULL				Cyp11A1 	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_279_2_271_s_287	15733658	In addition, the adult ovary gene set included all relevant steroidogenic regulators  and enzymes that are expressed in luteal cells and adult stroma (including steroidogenic  factor  SF1 (H3053B11, confirmatory data in  Fig. 4), which regulates transcription of all cytochrome  P450s; P450ssc/Cyp11A1 (H3094D01), catalyzing the conversion of cholesterol to pregnenolone;  steroidogenic acute regulatory protein StAR (H3097G04), which regulates accessibility  of cholesterol to P450ssc; P450c17/Cyp17 (H3018A11), a theca cell marker that catalyzes  the formation of dehydroepiandrosterone (DHEA) and is upregulated by Gdf9 in preantral  follicles (  Vitt et al., 2000); and two clones (H3059B01, H3070C08) for placental 3- -hydroxysteroid dehydrogenase  Hsd3b1 (see OMIM109715)).	transcription
52914	9	334826	6	NULL	NULL	0	NULL	P450ssc	NULL		is	NULL				H3094D01	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_279_2_271_s_287	15733658	In addition, the adult ovary gene set included all relevant steroidogenic regulators  and enzymes that are expressed in luteal cells and adult stroma (including steroidogenic  factor  SF1 (H3053B11, confirmatory data in  Fig. 4), which regulates transcription of all cytochrome  P450s; P450ssc/Cyp11A1 (H3094D01), catalyzing the conversion of cholesterol to pregnenolone;  steroidogenic acute regulatory protein StAR (H3097G04), which regulates accessibility  of cholesterol to P450ssc; P450c17/Cyp17 (H3018A11), a theca cell marker that catalyzes  the formation of dehydroepiandrosterone (DHEA) and is upregulated by Gdf9 in preantral  follicles (  Vitt et al., 2000); and two clones (H3059B01, H3070C08) for placental 3- -hydroxysteroid dehydrogenase  Hsd3b1 (see OMIM109715)).	transcription
52915	10	334826	6	NULL	NULL	0	NULL	StAR	NULL		is	NULL				steroidogenic acute regulatory protein	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_279_2_271_s_287	15733658	In addition, the adult ovary gene set included all relevant steroidogenic regulators  and enzymes that are expressed in luteal cells and adult stroma (including steroidogenic  factor  SF1 (H3053B11, confirmatory data in  Fig. 4), which regulates transcription of all cytochrome  P450s; P450ssc/Cyp11A1 (H3094D01), catalyzing the conversion of cholesterol to pregnenolone;  steroidogenic acute regulatory protein StAR (H3097G04), which regulates accessibility  of cholesterol to P450ssc; P450c17/Cyp17 (H3018A11), a theca cell marker that catalyzes  the formation of dehydroepiandrosterone (DHEA) and is upregulated by Gdf9 in preantral  follicles (  Vitt et al., 2000); and two clones (H3059B01, H3070C08) for placental 3- -hydroxysteroid dehydrogenase  Hsd3b1 (see OMIM109715)).	transcription
52916	11	334826	6	NULL	NULL	0	NULL	StAR	NULL		is	NULL				H3097G04	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_279_2_271_s_287	15733658	In addition, the adult ovary gene set included all relevant steroidogenic regulators  and enzymes that are expressed in luteal cells and adult stroma (including steroidogenic  factor  SF1 (H3053B11, confirmatory data in  Fig. 4), which regulates transcription of all cytochrome  P450s; P450ssc/Cyp11A1 (H3094D01), catalyzing the conversion of cholesterol to pregnenolone;  steroidogenic acute regulatory protein StAR (H3097G04), which regulates accessibility  of cholesterol to P450ssc; P450c17/Cyp17 (H3018A11), a theca cell marker that catalyzes  the formation of dehydroepiandrosterone (DHEA) and is upregulated by Gdf9 in preantral  follicles (  Vitt et al., 2000); and two clones (H3059B01, H3070C08) for placental 3- -hydroxysteroid dehydrogenase  Hsd3b1 (see OMIM109715)).	transcription
52917	12	334826	6	NULL	NULL	0	NULL	cholesterol	NULL		is accessible to	NULL				P450ssc	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_279_2_271_s_287	15733658	In addition, the adult ovary gene set included all relevant steroidogenic regulators  and enzymes that are expressed in luteal cells and adult stroma (including steroidogenic  factor  SF1 (H3053B11, confirmatory data in  Fig. 4), which regulates transcription of all cytochrome  P450s; P450ssc/Cyp11A1 (H3094D01), catalyzing the conversion of cholesterol to pregnenolone;  steroidogenic acute regulatory protein StAR (H3097G04), which regulates accessibility  of cholesterol to P450ssc; P450c17/Cyp17 (H3018A11), a theca cell marker that catalyzes  the formation of dehydroepiandrosterone (DHEA) and is upregulated by Gdf9 in preantral  follicles (  Vitt et al., 2000); and two clones (H3059B01, H3070C08) for placental 3- -hydroxysteroid dehydrogenase  Hsd3b1 (see OMIM109715)).	transcription
52918	13	334826	6	NULL	NULL	0	NULL	StAR	NULL		catalyzes	NULL				statement 12	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_279_2_271_s_287	15733658	In addition, the adult ovary gene set included all relevant steroidogenic regulators  and enzymes that are expressed in luteal cells and adult stroma (including steroidogenic  factor  SF1 (H3053B11, confirmatory data in  Fig. 4), which regulates transcription of all cytochrome  P450s; P450ssc/Cyp11A1 (H3094D01), catalyzing the conversion of cholesterol to pregnenolone;  steroidogenic acute regulatory protein StAR (H3097G04), which regulates accessibility  of cholesterol to P450ssc; P450c17/Cyp17 (H3018A11), a theca cell marker that catalyzes  the formation of dehydroepiandrosterone (DHEA) and is upregulated by Gdf9 in preantral  follicles (  Vitt et al., 2000); and two clones (H3059B01, H3070C08) for placental 3- -hydroxysteroid dehydrogenase  Hsd3b1 (see OMIM109715)).	transcription
52919	14	334826	6	NULL	NULL	0	NULL	P450c17	NULL		is	NULL				Cyp17	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_279_2_271_s_287	15733658	In addition, the adult ovary gene set included all relevant steroidogenic regulators  and enzymes that are expressed in luteal cells and adult stroma (including steroidogenic  factor  SF1 (H3053B11, confirmatory data in  Fig. 4), which regulates transcription of all cytochrome  P450s; P450ssc/Cyp11A1 (H3094D01), catalyzing the conversion of cholesterol to pregnenolone;  steroidogenic acute regulatory protein StAR (H3097G04), which regulates accessibility  of cholesterol to P450ssc; P450c17/Cyp17 (H3018A11), a theca cell marker that catalyzes  the formation of dehydroepiandrosterone (DHEA) and is upregulated by Gdf9 in preantral  follicles (  Vitt et al., 2000); and two clones (H3059B01, H3070C08) for placental 3- -hydroxysteroid dehydrogenase  Hsd3b1 (see OMIM109715)).	transcription
52921	15	334826	6	NULL	NULL	0	NULL	DHEA	NULL		is	NULL				dehydroepiandrosterone 	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_279_2_271_s_287	15733658	In addition, the adult ovary gene set included all relevant steroidogenic regulators  and enzymes that are expressed in luteal cells and adult stroma (including steroidogenic  factor  SF1 (H3053B11, confirmatory data in  Fig. 4), which regulates transcription of all cytochrome  P450s; P450ssc/Cyp11A1 (H3094D01), catalyzing the conversion of cholesterol to pregnenolone;  steroidogenic acute regulatory protein StAR (H3097G04), which regulates accessibility  of cholesterol to P450ssc; P450c17/Cyp17 (H3018A11), a theca cell marker that catalyzes  the formation of dehydroepiandrosterone (DHEA) and is upregulated by Gdf9 in preantral  follicles (  Vitt et al., 2000); and two clones (H3059B01, H3070C08) for placental 3- -hydroxysteroid dehydrogenase  Hsd3b1 (see OMIM109715)).	transcription
52922	16	334826	6	NULL	NULL	0	NULL	P450c17	NULL		is a type of	NULL				theca cell marker	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_279_2_271_s_287	15733658	In addition, the adult ovary gene set included all relevant steroidogenic regulators  and enzymes that are expressed in luteal cells and adult stroma (including steroidogenic  factor  SF1 (H3053B11, confirmatory data in  Fig. 4), which regulates transcription of all cytochrome  P450s; P450ssc/Cyp11A1 (H3094D01), catalyzing the conversion of cholesterol to pregnenolone;  steroidogenic acute regulatory protein StAR (H3097G04), which regulates accessibility  of cholesterol to P450ssc; P450c17/Cyp17 (H3018A11), a theca cell marker that catalyzes  the formation of dehydroepiandrosterone (DHEA) and is upregulated by Gdf9 in preantral  follicles (  Vitt et al., 2000); and two clones (H3059B01, H3070C08) for placental 3- -hydroxysteroid dehydrogenase  Hsd3b1 (see OMIM109715)).	transcription
52923	17	334826	6	NULL	NULL	0	NULL	P450c17	NULL		catalyzes	NULL				DHEA	NULL	formation of			NULL		0	NULL	NULL	NULL	gw70_devbiol_279_2_271_s_287	15733658	In addition, the adult ovary gene set included all relevant steroidogenic regulators  and enzymes that are expressed in luteal cells and adult stroma (including steroidogenic  factor  SF1 (H3053B11, confirmatory data in  Fig. 4), which regulates transcription of all cytochrome  P450s; P450ssc/Cyp11A1 (H3094D01), catalyzing the conversion of cholesterol to pregnenolone;  steroidogenic acute regulatory protein StAR (H3097G04), which regulates accessibility  of cholesterol to P450ssc; P450c17/Cyp17 (H3018A11), a theca cell marker that catalyzes  the formation of dehydroepiandrosterone (DHEA) and is upregulated by Gdf9 in preantral  follicles (  Vitt et al., 2000); and two clones (H3059B01, H3070C08) for placental 3- -hydroxysteroid dehydrogenase  Hsd3b1 (see OMIM109715)).	transcription
52924	18	334826	6	NULL	NULL	0	NULL	P450c17	NULL		is	NULL				H3018A11	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_279_2_271_s_287	15733658	In addition, the adult ovary gene set included all relevant steroidogenic regulators  and enzymes that are expressed in luteal cells and adult stroma (including steroidogenic  factor  SF1 (H3053B11, confirmatory data in  Fig. 4), which regulates transcription of all cytochrome  P450s; P450ssc/Cyp11A1 (H3094D01), catalyzing the conversion of cholesterol to pregnenolone;  steroidogenic acute regulatory protein StAR (H3097G04), which regulates accessibility  of cholesterol to P450ssc; P450c17/Cyp17 (H3018A11), a theca cell marker that catalyzes  the formation of dehydroepiandrosterone (DHEA) and is upregulated by Gdf9 in preantral  follicles (  Vitt et al., 2000); and two clones (H3059B01, H3070C08) for placental 3- -hydroxysteroid dehydrogenase  Hsd3b1 (see OMIM109715)).	transcription
52925	19	334826	6	NULL	NULL	0	NULL	Gdf9	NULL		upregulates	NULL				p450c17	NULL				NULL	preantral follicles	0	NULL	NULL	NULL	gw70_devbiol_279_2_271_s_287	15733658	In addition, the adult ovary gene set included all relevant steroidogenic regulators  and enzymes that are expressed in luteal cells and adult stroma (including steroidogenic  factor  SF1 (H3053B11, confirmatory data in  Fig. 4), which regulates transcription of all cytochrome  P450s; P450ssc/Cyp11A1 (H3094D01), catalyzing the conversion of cholesterol to pregnenolone;  steroidogenic acute regulatory protein StAR (H3097G04), which regulates accessibility  of cholesterol to P450ssc; P450c17/Cyp17 (H3018A11), a theca cell marker that catalyzes  the formation of dehydroepiandrosterone (DHEA) and is upregulated by Gdf9 in preantral  follicles (  Vitt et al., 2000); and two clones (H3059B01, H3070C08) for placental 3- -hydroxysteroid dehydrogenase  Hsd3b1 (see OMIM109715)).	transcription
51600	1	334827	5	NULL	NULL	0	NULL	L-glutamine	NULL	hydrolysis of	produce	NULL				ammonia	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_27_24579_s_145	11967268	Interdomain Channeling and Synchronization--  During catalysis of Fd-GltS, ammonia produced by L-glutamine hydrolysis is channeled to the 2-oxoglutarate-binding site, in which 2-iminoglutarate is formed.	transcription
51601	2	334827	5	NULL	NULL	0	NULL	statement 1	NULL		occurs during	NULL				Fd-GltS	NULL	catalysis of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_27_24579_s_145	11967268	Interdomain Channeling and Synchronization--  During catalysis of Fd-GltS, ammonia produced by L-glutamine hydrolysis is channeled to the 2-oxoglutarate-binding site, in which 2-iminoglutarate is formed.	transcription
51602	3	334827	5	NULL	NULL	0	NULL	ammonia	NULL		is channeled to	NULL					NULL		2-oxoglutarate-binding site		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_27_24579_s_145	11967268	Interdomain Channeling and Synchronization--  During catalysis of Fd-GltS, ammonia produced by L-glutamine hydrolysis is channeled to the 2-oxoglutarate-binding site, in which 2-iminoglutarate is formed.	transcription
51603	4	334827	5	NULL	NULL	0	NULL	2-iminoglutarate	NULL		is formed in	NULL					NULL		2-oxoglutarate-binding site		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_27_24579_s_145	11967268	Interdomain Channeling and Synchronization--  During catalysis of Fd-GltS, ammonia produced by L-glutamine hydrolysis is channeled to the 2-oxoglutarate-binding site, in which 2-iminoglutarate is formed.	transcription
51963	1	334827	6	NULL	NULL	0	NULL	L-glutamine	NULL	hydrolysis of	produces	NULL				ammonia	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_27_24579_s_145	11967268	Interdomain Channeling and Synchronization--  During catalysis of Fd-GltS, ammonia produced by L-glutamine hydrolysis is channeled to the 2-oxoglutarate-binding site, in which 2-iminoglutarate is formed.	transcription
51964	2	334827	6	NULL	NULL	0	NULL	statement 1	NULL		occurs during	NULL				Fd-GltS	NULL	catalysis of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_27_24579_s_145	11967268	Interdomain Channeling and Synchronization--  During catalysis of Fd-GltS, ammonia produced by L-glutamine hydrolysis is channeled to the 2-oxoglutarate-binding site, in which 2-iminoglutarate is formed.	transcription
51965	3	334827	6	NULL	NULL	0	NULL	ammonia	NULL		is channeled to	NULL					NULL		2-oxoglutarate-binding site		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_27_24579_s_145	11967268	Interdomain Channeling and Synchronization--  During catalysis of Fd-GltS, ammonia produced by L-glutamine hydrolysis is channeled to the 2-oxoglutarate-binding site, in which 2-iminoglutarate is formed.	transcription
51966	4	334827	6	NULL	NULL	0	NULL	2-iminoglutarate	NULL		is formed in	NULL					NULL		2-oxoglutarate-binding site		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_27_24579_s_145	11967268	Interdomain Channeling and Synchronization--  During catalysis of Fd-GltS, ammonia produced by L-glutamine hydrolysis is channeled to the 2-oxoglutarate-binding site, in which 2-iminoglutarate is formed.	transcription
52026	1	334828	5	NULL	NULL	0	NULL	ammonia	NULL		is added to	NULL				2-oxoglutarate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_27_24579_s_76	11967268	In the FMN-binding domain the 2-iminoglutarate intermediate, formed upon the addition of ammonia onto 2-oxoglutarate, is reduced by the FMN cofactor producing the second molecule of L-glutamate (Scheme 1).	transcription
52027	2	334828	5	NULL	NULL	0	NULL	statement 1	NULL		forms	NULL				2-iminoglutarate intermediate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_27_24579_s_76	11967268	In the FMN-binding domain the 2-iminoglutarate intermediate, formed upon the addition of ammonia onto 2-oxoglutarate, is reduced by the FMN cofactor producing the second molecule of L-glutamate (Scheme 1).	transcription
52028	3	334828	5	NULL	NULL	0	NULL	2-iminoglutarate intermediate	NULL		is reduced by	NULL				FMN cofactor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_27_24579_s_76	11967268	In the FMN-binding domain the 2-iminoglutarate intermediate, formed upon the addition of ammonia onto 2-oxoglutarate, is reduced by the FMN cofactor producing the second molecule of L-glutamate (Scheme 1).	transcription
52029	4	334828	5	NULL	NULL	0	NULL	statement 3	NULL		produce	NULL				L-glutamate	NULL	second molecule of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_27_24579_s_76	11967268	In the FMN-binding domain the 2-iminoglutarate intermediate, formed upon the addition of ammonia onto 2-oxoglutarate, is reduced by the FMN cofactor producing the second molecule of L-glutamate (Scheme 1).	transcription
51997	1	334828	6	NULL	NULL	0	NULL	ammonia	NULL		is added onto	NULL				2-oxoglutarate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_27_24579_s_76	11967268	In the FMN-binding domain the 2-iminoglutarate intermediate, formed upon the addition of ammonia onto 2-oxoglutarate, is reduced by the FMN cofactor producing the second molecule of L-glutamate (Scheme 1).	transcription
51998	2	334828	6	NULL	NULL	0	NULL	statement 1	NULL		forms	NULL				2-iminoglutarate intermediate	NULL		FMN-binding domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_27_24579_s_76	11967268	In the FMN-binding domain the 2-iminoglutarate intermediate, formed upon the addition of ammonia onto 2-oxoglutarate, is reduced by the FMN cofactor producing the second molecule of L-glutamate (Scheme 1).	transcription
51999	3	334828	6	NULL	NULL	0	NULL	FMN cofactor	NULL		produces	NULL				L-glutamate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_27_24579_s_76	11967268	In the FMN-binding domain the 2-iminoglutarate intermediate, formed upon the addition of ammonia onto 2-oxoglutarate, is reduced by the FMN cofactor producing the second molecule of L-glutamate (Scheme 1).	transcription
52000	4	334828	6	NULL	NULL	0	NULL	statement 2	NULL		is reduced by	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_27_24579_s_76	11967268	In the FMN-binding domain the 2-iminoglutarate intermediate, formed upon the addition of ammonia onto 2-oxoglutarate, is reduced by the FMN cofactor producing the second molecule of L-glutamate (Scheme 1).	transcription
51604	1	334830	5	NULL	NULL	0	NULL	oxoglutarate/fumarate exchange reaction	NULL		is catalyzed by	NULL				ACR1	NULL	reconstituted			NULL		0	NULL	NULL	NULL	gw60_febslett_417_1_114_s_86	9395087	The [14]oxoglutarate/fumarate exchange reaction catalysed by reconstituted ACR1 was inhibited by sulphydryl reagents (mersalyl,  p-chloromercuribenzene sulphonate and mercuric chloride), by pyridoxal 5-phosphate and by bathophenanthroline (see  Table 2).	transcription
51605	2	334830	5	NULL	NULL	0	NULL	mersalyl	NULL		is a type of	NULL				sulphydryl reagents	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_417_1_114_s_86	9395087	The [14]oxoglutarate/fumarate exchange reaction catalysed by reconstituted ACR1 was inhibited by sulphydryl reagents (mersalyl,  p-chloromercuribenzene sulphonate and mercuric chloride), by pyridoxal 5-phosphate and by bathophenanthroline (see  Table 2).	transcription
51606	3	334830	5	NULL	NULL	0	NULL	mersalyl	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_417_1_114_s_86	9395087	The [14]oxoglutarate/fumarate exchange reaction catalysed by reconstituted ACR1 was inhibited by sulphydryl reagents (mersalyl,  p-chloromercuribenzene sulphonate and mercuric chloride), by pyridoxal 5-phosphate and by bathophenanthroline (see  Table 2).	transcription
51607	4	334830	5	NULL	NULL	0	NULL	p-chloromercuribenzene sulphonate	NULL		is a type of	NULL				sulphydryl reagents	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_417_1_114_s_86	9395087	The [14]oxoglutarate/fumarate exchange reaction catalysed by reconstituted ACR1 was inhibited by sulphydryl reagents (mersalyl,  p-chloromercuribenzene sulphonate and mercuric chloride), by pyridoxal 5-phosphate and by bathophenanthroline (see  Table 2).	transcription
51608	5	334830	5	NULL	NULL	0	NULL	p-chloromercuribenzene sulphonate	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_417_1_114_s_86	9395087	The [14]oxoglutarate/fumarate exchange reaction catalysed by reconstituted ACR1 was inhibited by sulphydryl reagents (mersalyl,  p-chloromercuribenzene sulphonate and mercuric chloride), by pyridoxal 5-phosphate and by bathophenanthroline (see  Table 2).	transcription
51609	6	334830	5	NULL	NULL	0	NULL	mercuric chloride	NULL		is a type of	NULL				sulphydryl reagents	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_417_1_114_s_86	9395087	The [14]oxoglutarate/fumarate exchange reaction catalysed by reconstituted ACR1 was inhibited by sulphydryl reagents (mersalyl,  p-chloromercuribenzene sulphonate and mercuric chloride), by pyridoxal 5-phosphate and by bathophenanthroline (see  Table 2).	transcription
51610	7	334830	5	NULL	NULL	0	NULL	mercuric chloride	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_417_1_114_s_86	9395087	The [14]oxoglutarate/fumarate exchange reaction catalysed by reconstituted ACR1 was inhibited by sulphydryl reagents (mersalyl,  p-chloromercuribenzene sulphonate and mercuric chloride), by pyridoxal 5-phosphate and by bathophenanthroline (see  Table 2).	transcription
51611	8	334830	5	NULL	NULL	0	NULL	pyridoxal 5-phosphate	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_417_1_114_s_86	9395087	The [14]oxoglutarate/fumarate exchange reaction catalysed by reconstituted ACR1 was inhibited by sulphydryl reagents (mersalyl,  p-chloromercuribenzene sulphonate and mercuric chloride), by pyridoxal 5-phosphate and by bathophenanthroline (see  Table 2).	transcription
51612	9	334830	5	NULL	NULL	0	NULL	bathophenanthroline	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_417_1_114_s_86	9395087	The [14]oxoglutarate/fumarate exchange reaction catalysed by reconstituted ACR1 was inhibited by sulphydryl reagents (mersalyl,  p-chloromercuribenzene sulphonate and mercuric chloride), by pyridoxal 5-phosphate and by bathophenanthroline (see  Table 2).	transcription
52001	1	334830	6	NULL	NULL	0	NULL	ACR1	NULL	reconstituted	catalyzes	NULL				oxoglutarate/fumarate exchange reaction	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_417_1_114_s_86	9395087	The [14]oxoglutarate/fumarate exchange reaction catalysed by reconstituted ACR1 was inhibited by sulphydryl reagents (mersalyl,  p-chloromercuribenzene sulphonate and mercuric chloride), by pyridoxal 5-phosphate and by bathophenanthroline (see  Table 2).	transcription
52002	2	334830	6	NULL	NULL	0	NULL	mersalyl	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_417_1_114_s_86	9395087	The [14]oxoglutarate/fumarate exchange reaction catalysed by reconstituted ACR1 was inhibited by sulphydryl reagents (mersalyl,  p-chloromercuribenzene sulphonate and mercuric chloride), by pyridoxal 5-phosphate and by bathophenanthroline (see  Table 2).	transcription
52003	3	334830	6	NULL	NULL	0	NULL	p-chloromercuribenzene sulphonate	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_417_1_114_s_86	9395087	The [14]oxoglutarate/fumarate exchange reaction catalysed by reconstituted ACR1 was inhibited by sulphydryl reagents (mersalyl,  p-chloromercuribenzene sulphonate and mercuric chloride), by pyridoxal 5-phosphate and by bathophenanthroline (see  Table 2).	transcription
52004	4	334830	6	NULL	NULL	0	NULL	mercuric chloride	NULL		inhibits	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_417_1_114_s_86	9395087	The [14]oxoglutarate/fumarate exchange reaction catalysed by reconstituted ACR1 was inhibited by sulphydryl reagents (mersalyl,  p-chloromercuribenzene sulphonate and mercuric chloride), by pyridoxal 5-phosphate and by bathophenanthroline (see  Table 2).	transcription
52005	5	334830	6	NULL	NULL	0	NULL	mersalyl	NULL		is a type of	NULL				sulphydryl reagents	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_417_1_114_s_86	9395087	The [14]oxoglutarate/fumarate exchange reaction catalysed by reconstituted ACR1 was inhibited by sulphydryl reagents (mersalyl,  p-chloromercuribenzene sulphonate and mercuric chloride), by pyridoxal 5-phosphate and by bathophenanthroline (see  Table 2).	transcription
52006	6	334830	6	NULL	NULL	0	NULL	p-chloromercuribenzene sulphonate	NULL		is a type of	NULL				sulphydryl reagents	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_417_1_114_s_86	9395087	The [14]oxoglutarate/fumarate exchange reaction catalysed by reconstituted ACR1 was inhibited by sulphydryl reagents (mersalyl,  p-chloromercuribenzene sulphonate and mercuric chloride), by pyridoxal 5-phosphate and by bathophenanthroline (see  Table 2).	transcription
52007	7	334830	6	NULL	NULL	0	NULL	mercuric chloride	NULL		is a type of	NULL				sulphydryl reagents	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_417_1_114_s_86	9395087	The [14]oxoglutarate/fumarate exchange reaction catalysed by reconstituted ACR1 was inhibited by sulphydryl reagents (mersalyl,  p-chloromercuribenzene sulphonate and mercuric chloride), by pyridoxal 5-phosphate and by bathophenanthroline (see  Table 2).	transcription
51613	1	334831	5	NULL	NULL	0	NULL	fructose-6-phosphate specific enzyme	NULL		is a type of	NULL				phosphoketolases	NULL				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiollett_235_1_35_s_139	15158259	To date, two types of phosphoketolases have been described in  Bifidobacterium: a fructose-6-phosphate specific enzyme, which catalyzes the conversion of fructose-6-phosphate  to eritrose-4-phosphate and acetyl-phosphate, and a dual substrate xylulose-5-phosphate/fructose-6-phosphate  phosphoketolase, which can also act on xylulose-5-phosphate rendering acetyl-phosphate  and glyceraldehyde-3-phosphate [ 20 and   21].	transcription
51614	2	334831	5	NULL	NULL	0	NULL	fructose-6-phosphate	NULL		is converted to	NULL				eritrose-4-phosphate	NULL				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiollett_235_1_35_s_139	15158259	To date, two types of phosphoketolases have been described in  Bifidobacterium: a fructose-6-phosphate specific enzyme, which catalyzes the conversion of fructose-6-phosphate  to eritrose-4-phosphate and acetyl-phosphate, and a dual substrate xylulose-5-phosphate/fructose-6-phosphate  phosphoketolase, which can also act on xylulose-5-phosphate rendering acetyl-phosphate  and glyceraldehyde-3-phosphate [ 20 and   21].	transcription
51615	3	334831	5	NULL	NULL	0	NULL	fructose-6-phosphate	NULL		is converted to	NULL				acetyl-phosphate	NULL				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiollett_235_1_35_s_139	15158259	To date, two types of phosphoketolases have been described in  Bifidobacterium: a fructose-6-phosphate specific enzyme, which catalyzes the conversion of fructose-6-phosphate  to eritrose-4-phosphate and acetyl-phosphate, and a dual substrate xylulose-5-phosphate/fructose-6-phosphate  phosphoketolase, which can also act on xylulose-5-phosphate rendering acetyl-phosphate  and glyceraldehyde-3-phosphate [ 20 and   21].	transcription
51616	4	334831	5	NULL	NULL	0	NULL	fructose-6-phosphate specific enzyme	NULL	Bifidobacterium	catalyzes	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiollett_235_1_35_s_139	15158259	To date, two types of phosphoketolases have been described in  Bifidobacterium: a fructose-6-phosphate specific enzyme, which catalyzes the conversion of fructose-6-phosphate  to eritrose-4-phosphate and acetyl-phosphate, and a dual substrate xylulose-5-phosphate/fructose-6-phosphate  phosphoketolase, which can also act on xylulose-5-phosphate rendering acetyl-phosphate  and glyceraldehyde-3-phosphate [ 20 and   21].	transcription
51617	5	334831	5	NULL	NULL	0	NULL	fructose-6-phosphate specific enzyme	NULL	Bifidobacterium	catalyzes	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiollett_235_1_35_s_139	15158259	To date, two types of phosphoketolases have been described in  Bifidobacterium: a fructose-6-phosphate specific enzyme, which catalyzes the conversion of fructose-6-phosphate  to eritrose-4-phosphate and acetyl-phosphate, and a dual substrate xylulose-5-phosphate/fructose-6-phosphate  phosphoketolase, which can also act on xylulose-5-phosphate rendering acetyl-phosphate  and glyceraldehyde-3-phosphate [ 20 and   21].	transcription
51618	6	334831	5	NULL	NULL	0	NULL	xylulose-5-phosphate/fructose-6-phosphate phosphoketolase	NULL		is a type of	NULL				dual substrate	NULL				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiollett_235_1_35_s_139	15158259	To date, two types of phosphoketolases have been described in  Bifidobacterium: a fructose-6-phosphate specific enzyme, which catalyzes the conversion of fructose-6-phosphate  to eritrose-4-phosphate and acetyl-phosphate, and a dual substrate xylulose-5-phosphate/fructose-6-phosphate  phosphoketolase, which can also act on xylulose-5-phosphate rendering acetyl-phosphate  and glyceraldehyde-3-phosphate [ 20 and   21].	transcription
51619	7	334831	5	NULL	NULL	0	NULL	xylulose-5-phosphate/fructose-6-phosphate phosphoketolase	NULL	Bifidobacterium	acts on	NULL				xylulose-5-phosphate	NULL				NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiollett_235_1_35_s_139	15158259	To date, two types of phosphoketolases have been described in  Bifidobacterium: a fructose-6-phosphate specific enzyme, which catalyzes the conversion of fructose-6-phosphate  to eritrose-4-phosphate and acetyl-phosphate, and a dual substrate xylulose-5-phosphate/fructose-6-phosphate  phosphoketolase, which can also act on xylulose-5-phosphate rendering acetyl-phosphate  and glyceraldehyde-3-phosphate [ 20 and   21].	transcription
51620	8	334831	5	NULL	NULL	0	NULL	statement 7	NULL		renders	NULL				acetyl-phosphate	NULL				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiollett_235_1_35_s_139	15158259	To date, two types of phosphoketolases have been described in  Bifidobacterium: a fructose-6-phosphate specific enzyme, which catalyzes the conversion of fructose-6-phosphate  to eritrose-4-phosphate and acetyl-phosphate, and a dual substrate xylulose-5-phosphate/fructose-6-phosphate  phosphoketolase, which can also act on xylulose-5-phosphate rendering acetyl-phosphate  and glyceraldehyde-3-phosphate [ 20 and   21].	transcription
51621	9	334831	5	NULL	NULL	0	NULL	statement 7	NULL		renders	NULL				glyceraldehyde-3-phosphate	NULL				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiollett_235_1_35_s_139	15158259	To date, two types of phosphoketolases have been described in  Bifidobacterium: a fructose-6-phosphate specific enzyme, which catalyzes the conversion of fructose-6-phosphate  to eritrose-4-phosphate and acetyl-phosphate, and a dual substrate xylulose-5-phosphate/fructose-6-phosphate  phosphoketolase, which can also act on xylulose-5-phosphate rendering acetyl-phosphate  and glyceraldehyde-3-phosphate [ 20 and   21].	transcription
52926	1	334831	6	NULL	NULL	0	NULL	fructose-6-phosphate	NULL		is converted to	NULL				eritrose-4-phosphate	NULL				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiollett_235_1_35_s_139	15158259	To date, two types of phosphoketolases have been described in  Bifidobacterium: a fructose-6-phosphate specific enzyme, which catalyzes the conversion of fructose-6-phosphate  to eritrose-4-phosphate and acetyl-phosphate, and a dual substrate xylulose-5-phosphate/fructose-6-phosphate  phosphoketolase, which can also act on xylulose-5-phosphate rendering acetyl-phosphate  and glyceraldehyde-3-phosphate [ 20 and   21].	transcription
52927	2	334831	6	NULL	NULL	0	NULL	fructose-6-phosphate	NULL		is converted to	NULL				acetyl-phosphate	NULL				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiollett_235_1_35_s_139	15158259	To date, two types of phosphoketolases have been described in  Bifidobacterium: a fructose-6-phosphate specific enzyme, which catalyzes the conversion of fructose-6-phosphate  to eritrose-4-phosphate and acetyl-phosphate, and a dual substrate xylulose-5-phosphate/fructose-6-phosphate  phosphoketolase, which can also act on xylulose-5-phosphate rendering acetyl-phosphate  and glyceraldehyde-3-phosphate [ 20 and   21].	transcription
52928	3	334831	6	NULL	NULL	0	NULL	statement 1	NULL		occurs simultaneously with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiollett_235_1_35_s_139	15158259	To date, two types of phosphoketolases have been described in  Bifidobacterium: a fructose-6-phosphate specific enzyme, which catalyzes the conversion of fructose-6-phosphate  to eritrose-4-phosphate and acetyl-phosphate, and a dual substrate xylulose-5-phosphate/fructose-6-phosphate  phosphoketolase, which can also act on xylulose-5-phosphate rendering acetyl-phosphate  and glyceraldehyde-3-phosphate [ 20 and   21].	transcription
52929	4	334831	6	NULL	NULL	0	NULL	fructose-6-phosphate	NULL		catalyzes	NULL				statement 1	NULL				NULL	Bifidobacterium	NULL	NULL	NULL	NULL	gw70_femsmicrobiollett_235_1_35_s_139	15158259	To date, two types of phosphoketolases have been described in  Bifidobacterium: a fructose-6-phosphate specific enzyme, which catalyzes the conversion of fructose-6-phosphate  to eritrose-4-phosphate and acetyl-phosphate, and a dual substrate xylulose-5-phosphate/fructose-6-phosphate  phosphoketolase, which can also act on xylulose-5-phosphate rendering acetyl-phosphate  and glyceraldehyde-3-phosphate [ 20 and   21].	transcription
52930	5	334831	6	NULL	NULL	0	NULL	fructose-6-phosphate	NULL		catalyzes	NULL				statement 2	NULL				NULL	Bifidobacterium	0	NULL	NULL	NULL	gw70_femsmicrobiollett_235_1_35_s_139	15158259	To date, two types of phosphoketolases have been described in  Bifidobacterium: a fructose-6-phosphate specific enzyme, which catalyzes the conversion of fructose-6-phosphate  to eritrose-4-phosphate and acetyl-phosphate, and a dual substrate xylulose-5-phosphate/fructose-6-phosphate  phosphoketolase, which can also act on xylulose-5-phosphate rendering acetyl-phosphate  and glyceraldehyde-3-phosphate [ 20 and   21].	transcription
52931	6	334831	6	NULL	NULL	0	NULL	xylulose-5-phosphate	NULL		is converted to	NULL				acetyl-phosphate	NULL				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiollett_235_1_35_s_139	15158259	To date, two types of phosphoketolases have been described in  Bifidobacterium: a fructose-6-phosphate specific enzyme, which catalyzes the conversion of fructose-6-phosphate  to eritrose-4-phosphate and acetyl-phosphate, and a dual substrate xylulose-5-phosphate/fructose-6-phosphate  phosphoketolase, which can also act on xylulose-5-phosphate rendering acetyl-phosphate  and glyceraldehyde-3-phosphate [ 20 and   21].	transcription
52932	7	334831	6	NULL	NULL	0	NULL	xylulose-5-phosphate	NULL		is converted to	NULL				glyceraldehyde-3-phosphate	NULL				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiollett_235_1_35_s_139	15158259	To date, two types of phosphoketolases have been described in  Bifidobacterium: a fructose-6-phosphate specific enzyme, which catalyzes the conversion of fructose-6-phosphate  to eritrose-4-phosphate and acetyl-phosphate, and a dual substrate xylulose-5-phosphate/fructose-6-phosphate  phosphoketolase, which can also act on xylulose-5-phosphate rendering acetyl-phosphate  and glyceraldehyde-3-phosphate [ 20 and   21].	transcription
52933	8	334831	6	NULL	NULL	0	NULL	statement 6	NULL		occurs simultaneously with	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiollett_235_1_35_s_139	15158259	To date, two types of phosphoketolases have been described in  Bifidobacterium: a fructose-6-phosphate specific enzyme, which catalyzes the conversion of fructose-6-phosphate  to eritrose-4-phosphate and acetyl-phosphate, and a dual substrate xylulose-5-phosphate/fructose-6-phosphate  phosphoketolase, which can also act on xylulose-5-phosphate rendering acetyl-phosphate  and glyceraldehyde-3-phosphate [ 20 and   21].	transcription
52934	9	334831	6	NULL	NULL	0	NULL	xylulose-5-phosphate/fructose-6-phosphate phosphoketolase	NULL		catalyzes	NULL				statement 6	NULL				NULL	Bifidobacterium	NULL	NULL	NULL	NULL	gw70_femsmicrobiollett_235_1_35_s_139	15158259	To date, two types of phosphoketolases have been described in  Bifidobacterium: a fructose-6-phosphate specific enzyme, which catalyzes the conversion of fructose-6-phosphate  to eritrose-4-phosphate and acetyl-phosphate, and a dual substrate xylulose-5-phosphate/fructose-6-phosphate  phosphoketolase, which can also act on xylulose-5-phosphate rendering acetyl-phosphate  and glyceraldehyde-3-phosphate [ 20 and   21].	transcription
52935	10	334831	6	NULL	NULL	0	NULL	xylulose-5-phosphate/fructose-6-phosphate phosphoketolase	NULL		catalyzes	NULL				statement 7	NULL				NULL	Bifidobacterium	NULL	NULL	NULL	NULL	gw70_femsmicrobiollett_235_1_35_s_139	15158259	To date, two types of phosphoketolases have been described in  Bifidobacterium: a fructose-6-phosphate specific enzyme, which catalyzes the conversion of fructose-6-phosphate  to eritrose-4-phosphate and acetyl-phosphate, and a dual substrate xylulose-5-phosphate/fructose-6-phosphate  phosphoketolase, which can also act on xylulose-5-phosphate rendering acetyl-phosphate  and glyceraldehyde-3-phosphate [ 20 and   21].	transcription
51622	1	334832	5	NULL	NULL	0	NULL	fructose-1-phosphate	NULL	presence of	activates	NULL				glyceraldehyde-3-phosphate dehydrogenase	NULL	T. tenax			NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_8_2836_s_185	16585745	T. tenax glyceraldehyde-3-phosphate dehydrogenase was found to be activated by the presence of fructose-1-phosphate and fructose-6-phosphate ( ); however, activation of  M. jannaschii lactaldehyde dehydrogenase by these sugar-phosphates was not observed.	transcription
51623	2	334832	5	NULL	NULL	0	NULL	fructose-6-phosphate	NULL	presence of	activates	NULL				glyceraldehyde-3-phosphate dehydrogenase	NULL	T. tenax			NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_8_2836_s_185	16585745	T. tenax glyceraldehyde-3-phosphate dehydrogenase was found to be activated by the presence of fructose-1-phosphate and fructose-6-phosphate ( ); however, activation of  M. jannaschii lactaldehyde dehydrogenase by these sugar-phosphates was not observed.	transcription
51624	3	334832	5	NULL	NULL	0	NULL	fructose-1-phosphate	NULL	presence of	does not activate	NULL				lactaldehyde dehydrogenase	NULL	M. jannaschii 			NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_8_2836_s_185	16585745	T. tenax glyceraldehyde-3-phosphate dehydrogenase was found to be activated by the presence of fructose-1-phosphate and fructose-6-phosphate ( ); however, activation of  M. jannaschii lactaldehyde dehydrogenase by these sugar-phosphates was not observed.	transcription
51625	4	334832	5	NULL	NULL	0	NULL	fructose-6-phosphate	NULL	presence of	does not activate	NULL				lactaldehyde dehydrogenase	NULL	M. jannaschii			NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_8_2836_s_185	16585745	T. tenax glyceraldehyde-3-phosphate dehydrogenase was found to be activated by the presence of fructose-1-phosphate and fructose-6-phosphate ( ); however, activation of  M. jannaschii lactaldehyde dehydrogenase by these sugar-phosphates was not observed.	transcription
52008	1	334832	6	NULL	NULL	0	NULL	glyceraldehyde-3-phosphate dehydrogenase	NULL	T. tenax	is activated by	NULL				fructose-1-phosphate	NULL	presence of 			NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_8_2836_s_185	16585745	T. tenax glyceraldehyde-3-phosphate dehydrogenase was found to be activated by the presence of fructose-1-phosphate and fructose-6-phosphate ( ); however, activation of  M. jannaschii lactaldehyde dehydrogenase by these sugar-phosphates was not observed.	transcription
52009	2	334832	6	NULL	NULL	0	NULL	glyceraldehyde-3-phosphate dehydrogenase	NULL	T. tenax	is activated by	NULL				fructose-6-phosphate	NULL	presence of 			NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_8_2836_s_185	16585745	T. tenax glyceraldehyde-3-phosphate dehydrogenase was found to be activated by the presence of fructose-1-phosphate and fructose-6-phosphate ( ); however, activation of  M. jannaschii lactaldehyde dehydrogenase by these sugar-phosphates was not observed.	transcription
52010	3	334832	6	NULL	NULL	0	NULL	lactaldehyde dehydrogenase	NULL	M. jannaschii	is not activated by	NULL				fructose-1-phosphate	NULL	presence of 			NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_8_2836_s_185	16585745	T. tenax glyceraldehyde-3-phosphate dehydrogenase was found to be activated by the presence of fructose-1-phosphate and fructose-6-phosphate ( ); however, activation of  M. jannaschii lactaldehyde dehydrogenase by these sugar-phosphates was not observed.	transcription
52011	4	334832	6	NULL	NULL	0	NULL	lactaldehyde dehydrogenase	NULL	M. jannaschii	is not activated by	NULL				fructose-6-phosphate	NULL	presence of 			NULL		0	NULL	NULL	NULL	gw70_jbacteriol_188_8_2836_s_185	16585745	T. tenax glyceraldehyde-3-phosphate dehydrogenase was found to be activated by the presence of fructose-1-phosphate and fructose-6-phosphate ( ); however, activation of  M. jannaschii lactaldehyde dehydrogenase by these sugar-phosphates was not observed.	transcription
51626	1	334833	5	NULL	NULL	0	NULL	hyperglycemia	NULL		induce	NULL				superoxide	NULL	overproduction of;;mitochondrial			NULL		0	NULL	NULL	NULL	gw60_pnas_97_22_12222_s_21	11050244	In the present study, we show that hyperglycemia-induced mitochondrial superoxide overproduction inhibits glyceraldehyde-3-phosphate dehydrogenase (GAPDH) activity and activates the hexosamine pathway, presumably by diverting the upstream metabolite fructose-6-phosphate from glycolysis to glucosamine formation.	transcription
51627	2	334833	5	NULL	NULL	0	NULL	statement 1	NULL		inhibit	NULL				GAPDH	NULL	activity of			NULL		0	NULL	NULL	NULL	gw60_pnas_97_22_12222_s_21	11050244	In the present study, we show that hyperglycemia-induced mitochondrial superoxide overproduction inhibits glyceraldehyde-3-phosphate dehydrogenase (GAPDH) activity and activates the hexosamine pathway, presumably by diverting the upstream metabolite fructose-6-phosphate from glycolysis to glucosamine formation.	transcription
51628	3	334833	5	NULL	NULL	0	NULL	GAPDH	NULL		is	NULL				glyceraldehyde-3-phosphate dehydrogenase	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_22_12222_s_21	11050244	In the present study, we show that hyperglycemia-induced mitochondrial superoxide overproduction inhibits glyceraldehyde-3-phosphate dehydrogenase (GAPDH) activity and activates the hexosamine pathway, presumably by diverting the upstream metabolite fructose-6-phosphate from glycolysis to glucosamine formation.	transcription
51629	4	334833	5	NULL	NULL	0	NULL	statement 1	NULL		activates	NULL				hexosamine pathway	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_22_12222_s_21	11050244	In the present study, we show that hyperglycemia-induced mitochondrial superoxide overproduction inhibits glyceraldehyde-3-phosphate dehydrogenase (GAPDH) activity and activates the hexosamine pathway, presumably by diverting the upstream metabolite fructose-6-phosphate from glycolysis to glucosamine formation.	transcription
51630	5	334833	5	NULL	NULL	0	NULL	fructose-6-phosphate	NULL		is a type of	NULL				upstream metabolite	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_22_12222_s_21	11050244	In the present study, we show that hyperglycemia-induced mitochondrial superoxide overproduction inhibits glyceraldehyde-3-phosphate dehydrogenase (GAPDH) activity and activates the hexosamine pathway, presumably by diverting the upstream metabolite fructose-6-phosphate from glycolysis to glucosamine formation.	transcription
51631	6	334833	5	NULL	NULL	0	NULL	fructose-6-phosphate	NULL		is diverted from	NULL				glycolysis	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_22_12222_s_21	11050244	In the present study, we show that hyperglycemia-induced mitochondrial superoxide overproduction inhibits glyceraldehyde-3-phosphate dehydrogenase (GAPDH) activity and activates the hexosamine pathway, presumably by diverting the upstream metabolite fructose-6-phosphate from glycolysis to glucosamine formation.	transcription
51632	7	334833	5	NULL	NULL	0	NULL	fructose-6-phosphate	NULL		is diverted to	NULL				glucosamine	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_pnas_97_22_12222_s_21	11050244	In the present study, we show that hyperglycemia-induced mitochondrial superoxide overproduction inhibits glyceraldehyde-3-phosphate dehydrogenase (GAPDH) activity and activates the hexosamine pathway, presumably by diverting the upstream metabolite fructose-6-phosphate from glycolysis to glucosamine formation.	transcription
51633	8	334833	5	NULL	NULL	0	NULL	statement 4	NULL		occurs by	NULL	presumably			statement 7	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_22_12222_s_21	11050244	In the present study, we show that hyperglycemia-induced mitochondrial superoxide overproduction inhibits glyceraldehyde-3-phosphate dehydrogenase (GAPDH) activity and activates the hexosamine pathway, presumably by diverting the upstream metabolite fructose-6-phosphate from glycolysis to glucosamine formation.	transcription
52012	1	334833	6	NULL	NULL	0	NULL	hyperglycemia	NULL		induces	NULL				mitochondrial superoxide	NULL	overproduction of 			NULL		0	NULL	NULL	NULL	gw60_pnas_97_22_12222_s_21	11050244	In the present study, we show that hyperglycemia-induced mitochondrial superoxide overproduction inhibits glyceraldehyde-3-phosphate dehydrogenase (GAPDH) activity and activates the hexosamine pathway, presumably by diverting the upstream metabolite fructose-6-phosphate from glycolysis to glucosamine formation.	transcription
52013	2	334833	6	NULL	NULL	0	NULL	statement 1	NULL		inhibits	NULL				GAPDH	NULL	activity of 			NULL		0	NULL	NULL	NULL	gw60_pnas_97_22_12222_s_21	11050244	In the present study, we show that hyperglycemia-induced mitochondrial superoxide overproduction inhibits glyceraldehyde-3-phosphate dehydrogenase (GAPDH) activity and activates the hexosamine pathway, presumably by diverting the upstream metabolite fructose-6-phosphate from glycolysis to glucosamine formation.	transcription
52014	3	334833	6	NULL	NULL	0	NULL	GAPDH	NULL		is	NULL				glyceraldehyde-3-phosphate dehydrogenase 	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_22_12222_s_21	11050244	In the present study, we show that hyperglycemia-induced mitochondrial superoxide overproduction inhibits glyceraldehyde-3-phosphate dehydrogenase (GAPDH) activity and activates the hexosamine pathway, presumably by diverting the upstream metabolite fructose-6-phosphate from glycolysis to glucosamine formation.	transcription
52015	4	334833	6	NULL	NULL	0	NULL	statement 1	NULL		activates	NULL				hexosamine pathway	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_22_12222_s_21	11050244	In the present study, we show that hyperglycemia-induced mitochondrial superoxide overproduction inhibits glyceraldehyde-3-phosphate dehydrogenase (GAPDH) activity and activates the hexosamine pathway, presumably by diverting the upstream metabolite fructose-6-phosphate from glycolysis to glucosamine formation.	transcription
52016	5	334833	6	NULL	NULL	0	NULL	fructose-6-phosphate	NULL		is diverted to	NULL				glucosamine	NULL	formation of 			NULL		0	NULL	NULL	NULL	gw60_pnas_97_22_12222_s_21	11050244	In the present study, we show that hyperglycemia-induced mitochondrial superoxide overproduction inhibits glyceraldehyde-3-phosphate dehydrogenase (GAPDH) activity and activates the hexosamine pathway, presumably by diverting the upstream metabolite fructose-6-phosphate from glycolysis to glucosamine formation.	transcription
52017	6	334833	6	NULL	NULL	0	NULL	statement 4	NULL		occurs by	NULL	presumably			statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_22_12222_s_21	11050244	In the present study, we show that hyperglycemia-induced mitochondrial superoxide overproduction inhibits glyceraldehyde-3-phosphate dehydrogenase (GAPDH) activity and activates the hexosamine pathway, presumably by diverting the upstream metabolite fructose-6-phosphate from glycolysis to glucosamine formation.	transcription
51634	1	334834	5	NULL	NULL	0	NULL	N, N-dimethylglycine	NULL		does not inhibit	NULL				betaine	NULL	transport of			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_17_5020_s_77	10940053	N, N-dimethylglycine did not inhibit [14]betaine transport (Table  1).	transcription
52018	1	334834	6	NULL	NULL	0	NULL	N, N-dimethylglycine	NULL		does not inhibit	NULL				betaine	NULL	transport of 			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_17_5020_s_77	10940053	N, N-dimethylglycine did not inhibit [14]betaine transport (Table  1).	transcription
52030	1	334835	5	NULL	NULL	0	NULL	glycine	NULL		is methylated to	NULL				sarcosine	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_7_4932_s_26	12466265	One of gene products catalyzed the methylation reactions of glycine and sarcosine to sarcosine and dimethylglycine, respectively (EcGSMT),1 whereas the other one catalyzed the methylations of sarcosine and dimethylglycine to dimethylglycine and betaine, respectively (EcSDMT) ( ,  ).	transcription
52031	2	334835	5	NULL	NULL	0	NULL	EcGSMT	NULL		catalyzes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_7_4932_s_26	12466265	One of gene products catalyzed the methylation reactions of glycine and sarcosine to sarcosine and dimethylglycine, respectively (EcGSMT),1 whereas the other one catalyzed the methylations of sarcosine and dimethylglycine to dimethylglycine and betaine, respectively (EcSDMT) ( ,  ).	transcription
52032	3	334835	5	NULL	NULL	0	NULL	sarcosine	NULL		is methylated to	NULL				dimethylglycine	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_7_4932_s_26	12466265	One of gene products catalyzed the methylation reactions of glycine and sarcosine to sarcosine and dimethylglycine, respectively (EcGSMT),1 whereas the other one catalyzed the methylations of sarcosine and dimethylglycine to dimethylglycine and betaine, respectively (EcSDMT) ( ,  ).	transcription
52033	4	334835	5	NULL	NULL	0	NULL	EcGSMT	NULL		catalyzes	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_7_4932_s_26	12466265	One of gene products catalyzed the methylation reactions of glycine and sarcosine to sarcosine and dimethylglycine, respectively (EcGSMT),1 whereas the other one catalyzed the methylations of sarcosine and dimethylglycine to dimethylglycine and betaine, respectively (EcSDMT) ( ,  ).	transcription
52034	5	334835	5	NULL	NULL	0	NULL	EcSDMT	NULL		catalyzes	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_7_4932_s_26	12466265	One of gene products catalyzed the methylation reactions of glycine and sarcosine to sarcosine and dimethylglycine, respectively (EcGSMT),1 whereas the other one catalyzed the methylations of sarcosine and dimethylglycine to dimethylglycine and betaine, respectively (EcSDMT) ( ,  ).	transcription
52035	6	334835	5	NULL	NULL	0	NULL	dimethylglycine	NULL		is methylated to	NULL				betaine	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_7_4932_s_26	12466265	One of gene products catalyzed the methylation reactions of glycine and sarcosine to sarcosine and dimethylglycine, respectively (EcGSMT),1 whereas the other one catalyzed the methylations of sarcosine and dimethylglycine to dimethylglycine and betaine, respectively (EcSDMT) ( ,  ).	transcription
52036	7	334835	5	NULL	NULL	0	NULL	EcSDMT	NULL		catalyzes	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_7_4932_s_26	12466265	One of gene products catalyzed the methylation reactions of glycine and sarcosine to sarcosine and dimethylglycine, respectively (EcGSMT),1 whereas the other one catalyzed the methylations of sarcosine and dimethylglycine to dimethylglycine and betaine, respectively (EcSDMT) ( ,  ).	transcription
52019	1	334835	6	NULL	NULL	0	NULL	glycine	NULL		is methylated to 	NULL				sarcosine	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_7_4932_s_26	12466265	One of gene products catalyzed the methylation reactions of glycine and sarcosine to sarcosine and dimethylglycine, respectively (EcGSMT),1 whereas the other one catalyzed the methylations of sarcosine and dimethylglycine to dimethylglycine and betaine, respectively (EcSDMT) ( ,  ).	transcription
52020	2	334835	6	NULL	NULL	0	NULL	sarcosine	NULL		is methylated to 	NULL				dimethylglycine	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_7_4932_s_26	12466265	One of gene products catalyzed the methylation reactions of glycine and sarcosine to sarcosine and dimethylglycine, respectively (EcGSMT),1 whereas the other one catalyzed the methylations of sarcosine and dimethylglycine to dimethylglycine and betaine, respectively (EcSDMT) ( ,  ).	transcription
52021	3	334835	6	NULL	NULL	0	NULL	EcGSMT	NULL		catalyzes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_7_4932_s_26	12466265	One of gene products catalyzed the methylation reactions of glycine and sarcosine to sarcosine and dimethylglycine, respectively (EcGSMT),1 whereas the other one catalyzed the methylations of sarcosine and dimethylglycine to dimethylglycine and betaine, respectively (EcSDMT) ( ,  ).	transcription
52022	4	334835	6	NULL	NULL	0	NULL	EcGSMT	NULL		catalyzes	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_7_4932_s_26	12466265	One of gene products catalyzed the methylation reactions of glycine and sarcosine to sarcosine and dimethylglycine, respectively (EcGSMT),1 whereas the other one catalyzed the methylations of sarcosine and dimethylglycine to dimethylglycine and betaine, respectively (EcSDMT) ( ,  ).	transcription
52023	5	334835	6	NULL	NULL	0	NULL	dimethylglycine	NULL		is methylated to 	NULL				betaine	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_7_4932_s_26	12466265	One of gene products catalyzed the methylation reactions of glycine and sarcosine to sarcosine and dimethylglycine, respectively (EcGSMT),1 whereas the other one catalyzed the methylations of sarcosine and dimethylglycine to dimethylglycine and betaine, respectively (EcSDMT) ( ,  ).	transcription
52024	6	334835	6	NULL	NULL	0	NULL	EcSDMT	NULL		catalyzes	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_7_4932_s_26	12466265	One of gene products catalyzed the methylation reactions of glycine and sarcosine to sarcosine and dimethylglycine, respectively (EcGSMT),1 whereas the other one catalyzed the methylations of sarcosine and dimethylglycine to dimethylglycine and betaine, respectively (EcSDMT) ( ,  ).	transcription
52025	7	334835	6	NULL	NULL	0	NULL	EcSDMT	NULL		catalyzes	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_7_4932_s_26	12466265	One of gene products catalyzed the methylation reactions of glycine and sarcosine to sarcosine and dimethylglycine, respectively (EcGSMT),1 whereas the other one catalyzed the methylations of sarcosine and dimethylglycine to dimethylglycine and betaine, respectively (EcSDMT) ( ,  ).	transcription
51635	1	334836	5	NULL	NULL	0	NULL	AmT1	NULL		mediate	NULL				proline 	NULL	uptake of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_21_18373_s_174	11907031	Dimethylglycine, monomethylglycine, and GABA also showed less competition than did betaine for proline uptake mediated by AmT1.	transcription
51636	2	334836	5	NULL	NULL	0	NULL	AmT1	NULL		mediate	NULL				betaine	NULL	uptake of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_21_18373_s_174	11907031	Dimethylglycine, monomethylglycine, and GABA also showed less competition than did betaine for proline uptake mediated by AmT1.	transcription
51637	3	334836	5	NULL	NULL	0	NULL	statement 2	NULL		competes with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_21_18373_s_174	11907031	Dimethylglycine, monomethylglycine, and GABA also showed less competition than did betaine for proline uptake mediated by AmT1.	transcription
51638	4	334836	5	NULL	NULL	0	NULL	AmT1	NULL		mediate	NULL				GABA	NULL	uptake of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_21_18373_s_174	11907031	Dimethylglycine, monomethylglycine, and GABA also showed less competition than did betaine for proline uptake mediated by AmT1.	transcription
51639	5	334836	5	NULL	NULL	0	NULL	statement 4	NULL		competes with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_21_18373_s_174	11907031	Dimethylglycine, monomethylglycine, and GABA also showed less competition than did betaine for proline uptake mediated by AmT1.	transcription
51640	6	334836	5	NULL	NULL	0	NULL	AmT1	NULL		mediate	NULL				monomethylglycine	NULL	uptake of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_21_18373_s_174	11907031	Dimethylglycine, monomethylglycine, and GABA also showed less competition than did betaine for proline uptake mediated by AmT1.	transcription
51641	7	334836	5	NULL	NULL	0	NULL	statement 6	NULL		competes with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_21_18373_s_174	11907031	Dimethylglycine, monomethylglycine, and GABA also showed less competition than did betaine for proline uptake mediated by AmT1.	transcription
51642	8	334836	5	NULL	NULL	0	NULL	AmT1	NULL		mediate	NULL				Dimethylglycine	NULL	uptake of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_21_18373_s_174	11907031	Dimethylglycine, monomethylglycine, and GABA also showed less competition than did betaine for proline uptake mediated by AmT1.	transcription
51643	9	334836	5	NULL	NULL	0	NULL	statement 8	NULL		competes with	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_21_18373_s_174	11907031	Dimethylglycine, monomethylglycine, and GABA also showed less competition than did betaine for proline uptake mediated by AmT1.	transcription
51644	10	334836	5	NULL	NULL	0	NULL	statement 5	NULL		lesser than	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_21_18373_s_174	11907031	Dimethylglycine, monomethylglycine, and GABA also showed less competition than did betaine for proline uptake mediated by AmT1.	transcription
51645	11	334836	5	NULL	NULL	0	NULL	statement 7	NULL		lesser than	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_21_18373_s_174	11907031	Dimethylglycine, monomethylglycine, and GABA also showed less competition than did betaine for proline uptake mediated by AmT1.	transcription
51646	12	334836	5	NULL	NULL	0	NULL	statement 9	NULL		lesser than	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_21_18373_s_174	11907031	Dimethylglycine, monomethylglycine, and GABA also showed less competition than did betaine for proline uptake mediated by AmT1.	transcription
52112	1	334836	6	NULL	NULL	0	NULL	AmT1	NULL		mediates	NULL				proline	NULL	uptake of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_21_18373_s_174	11907031	Dimethylglycine, monomethylglycine, and GABA also showed less competition than did betaine for proline uptake mediated by AmT1.	transcription
51647	1	334837	5	NULL	NULL	0	NULL	glycine betaine	NULL		inhibit	NULL	effectively			PB	NULL	uptake of			NULL	betS mutant	NULL	NULL	NULL	NULL	gw70_jbacteriol_188_17_6308_s_183	16923898	In contrast, several other compounds (glycine betaine, gamma-butyrobetaine, choline,  N, N-dimethylglycine,  N-methylproline, and DMSA) effectively inhibited the uptake of PB in the  betS mutant.	transcription
51648	2	334837	5	NULL	NULL	0	NULL	gamma-butyrobetaine	NULL		inhibit	NULL	effectively			PB	NULL	uptake of			NULL	betS mutant	0	NULL	NULL	NULL	gw70_jbacteriol_188_17_6308_s_183	16923898	In contrast, several other compounds (glycine betaine, gamma-butyrobetaine, choline,  N, N-dimethylglycine,  N-methylproline, and DMSA) effectively inhibited the uptake of PB in the  betS mutant.	transcription
51649	3	334837	5	NULL	NULL	0	NULL	choline	NULL		inhibit	NULL	effectively			PB	NULL	uptake of			NULL	betS mutant	0	NULL	NULL	NULL	gw70_jbacteriol_188_17_6308_s_183	16923898	In contrast, several other compounds (glycine betaine, gamma-butyrobetaine, choline,  N, N-dimethylglycine,  N-methylproline, and DMSA) effectively inhibited the uptake of PB in the  betS mutant.	transcription
51650	4	334837	5	NULL	NULL	0	NULL	N, N-dimethylglycine	NULL		inhibit	NULL	effectively			PB	NULL	uptake of			NULL	betS mutant	0	NULL	NULL	NULL	gw70_jbacteriol_188_17_6308_s_183	16923898	In contrast, several other compounds (glycine betaine, gamma-butyrobetaine, choline,  N, N-dimethylglycine,  N-methylproline, and DMSA) effectively inhibited the uptake of PB in the  betS mutant.	transcription
51651	5	334837	5	NULL	NULL	0	NULL	N-methylproline	NULL		inhibit	NULL	effectively			PB	NULL	uptake of			NULL	betS mutant	0	NULL	NULL	NULL	gw70_jbacteriol_188_17_6308_s_183	16923898	In contrast, several other compounds (glycine betaine, gamma-butyrobetaine, choline,  N, N-dimethylglycine,  N-methylproline, and DMSA) effectively inhibited the uptake of PB in the  betS mutant.	transcription
51652	6	334837	5	NULL	NULL	0	NULL	DMSA	NULL		inhibit	NULL	effectively			PB	NULL	uptake of			NULL	betS mutant	0	NULL	NULL	NULL	gw70_jbacteriol_188_17_6308_s_183	16923898	In contrast, several other compounds (glycine betaine, gamma-butyrobetaine, choline,  N, N-dimethylglycine,  N-methylproline, and DMSA) effectively inhibited the uptake of PB in the  betS mutant.	transcription
52113	1	334837	6	NULL	NULL	0	NULL	glycine betaine	NULL		inhibits	NULL				PB	NULL	uptake of 			NULL	betS mutant	NULL	NULL	NULL	NULL	gw70_jbacteriol_188_17_6308_s_183	16923898	In contrast, several other compounds (glycine betaine, gamma-butyrobetaine, choline,  N, N-dimethylglycine,  N-methylproline, and DMSA) effectively inhibited the uptake of PB in the  betS mutant.	transcription
52114	2	334837	6	NULL	NULL	0	NULL	gamma-butyrobetaine	NULL		inhibits	NULL				PB	NULL	uptake of 			NULL	betS mutant	0	NULL	NULL	NULL	gw70_jbacteriol_188_17_6308_s_183	16923898	In contrast, several other compounds (glycine betaine, gamma-butyrobetaine, choline,  N, N-dimethylglycine,  N-methylproline, and DMSA) effectively inhibited the uptake of PB in the  betS mutant.	transcription
52115	3	334837	6	NULL	NULL	0	NULL	choline	NULL		inhibits	NULL				PB	NULL	uptake of 			NULL	betS mutant	0	NULL	NULL	NULL	gw70_jbacteriol_188_17_6308_s_183	16923898	In contrast, several other compounds (glycine betaine, gamma-butyrobetaine, choline,  N, N-dimethylglycine,  N-methylproline, and DMSA) effectively inhibited the uptake of PB in the  betS mutant.	transcription
52116	4	334837	6	NULL	NULL	0	NULL	N, N-dimethylglycine	NULL		inhibits	NULL				PB	NULL	uptake of 			NULL	betS mutant	0	NULL	NULL	NULL	gw70_jbacteriol_188_17_6308_s_183	16923898	In contrast, several other compounds (glycine betaine, gamma-butyrobetaine, choline,  N, N-dimethylglycine,  N-methylproline, and DMSA) effectively inhibited the uptake of PB in the  betS mutant.	transcription
52117	5	334837	6	NULL	NULL	0	NULL	N-methylproline	NULL		inhibits	NULL				PB	NULL	uptake of 			NULL	betS mutant	NULL	NULL	NULL	NULL	gw70_jbacteriol_188_17_6308_s_183	16923898	In contrast, several other compounds (glycine betaine, gamma-butyrobetaine, choline,  N, N-dimethylglycine,  N-methylproline, and DMSA) effectively inhibited the uptake of PB in the  betS mutant.	transcription
52118	6	334837	6	NULL	NULL	0	NULL	DMSA	NULL		inhibits	NULL				PB	NULL	uptake of 			NULL	betS mutant	0	NULL	NULL	NULL	gw70_jbacteriol_188_17_6308_s_183	16923898	In contrast, several other compounds (glycine betaine, gamma-butyrobetaine, choline,  N, N-dimethylglycine,  N-methylproline, and DMSA) effectively inhibited the uptake of PB in the  betS mutant.	transcription
51653	1	334838	5	NULL	NULL	0	NULL	betaine	NULL		is synthesized from	NULL				glycine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_29_22196_s_113	10896953	Further analysis of the reaction products by HPLC (Fig.  1 A) and activity measurement on sarcosine and dimethylglycine confirm that the organisms synthesize betaine from glycine in a three-step methylation reaction.	transcription
52119	1	334838	6	NULL	NULL	0	NULL	betaine	NULL		is synthesized from	NULL				glycine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_29_22196_s_113	10896953	Further analysis of the reaction products by HPLC (Fig.  1 A) and activity measurement on sarcosine and dimethylglycine confirm that the organisms synthesize betaine from glycine in a three-step methylation reaction.	transcription
51654	1	334839	5	NULL	NULL	0	NULL	dimethylglycine	NULL		inhibit	NULL	uncompetitively			BHMT	NULL	activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_37_22831_s_242	8798461	Kinetic studies using the purified porcine enzyme indicate that dimethylglycine inhibits BHMT activity uncompetitively when Hcy is varied at either subsaturating (25 muM) or saturating (250 muM) levels of betaine.	transcription
52120	1	334839	6	NULL	NULL	0	NULL	dimethylglycine	NULL		inhibits	NULL				BHMT	NULL	activity of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_37_22831_s_242	8798461	Kinetic studies using the purified porcine enzyme indicate that dimethylglycine inhibits BHMT activity uncompetitively when Hcy is varied at either subsaturating (25 muM) or saturating (250 muM) levels of betaine.	transcription
51655	1	334840	5	NULL	NULL	0	NULL	glucose	NULL		is converted to	NULL				glucosamine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29179_s_128	10924527	Several studies have clearly established that the conversion of glucose into glucosamine, which is catalyzed by glutamine:fructose-6-phosphate amidotransferase (GFAT, EC 2.6.	transcription
51656	2	334840	5	NULL	NULL	0	NULL	GFAT	NULL		is	NULL				glutamine:fructose-6-phosphate amidotransferase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29179_s_128	10924527	Several studies have clearly established that the conversion of glucose into glucosamine, which is catalyzed by glutamine:fructose-6-phosphate amidotransferase (GFAT, EC 2.6.	transcription
51657	3	334840	5	NULL	NULL	0	NULL	GFAT	NULL		catalyzes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29179_s_128	10924527	Several studies have clearly established that the conversion of glucose into glucosamine, which is catalyzed by glutamine:fructose-6-phosphate amidotransferase (GFAT, EC 2.6.	transcription
52121	1	334840	6	NULL	NULL	0	NULL	glucose	NULL		is converted to	NULL				glucosamine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29179_s_128	10924527	Several studies have clearly established that the conversion of glucose into glucosamine, which is catalyzed by glutamine:fructose-6-phosphate amidotransferase (GFAT, EC 2.6.	transcription
52122	2	334840	6	NULL	NULL	0	NULL	statement 1	NULL		is catalyzed by	NULL				GFAT	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29179_s_128	10924527	Several studies have clearly established that the conversion of glucose into glucosamine, which is catalyzed by glutamine:fructose-6-phosphate amidotransferase (GFAT, EC 2.6.	transcription
52123	3	334840	6	NULL	NULL	0	NULL	GFAT	NULL		is	NULL				glutamine:fructose-6-phosphate amidotransferase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29179_s_128	10924527	Several studies have clearly established that the conversion of glucose into glucosamine, which is catalyzed by glutamine:fructose-6-phosphate amidotransferase (GFAT, EC 2.6.	transcription
51658	1	334841	5	NULL	NULL	0	NULL	GFAT	NULL		is	NULL				glutamine:fructose-6-phosphate amidotransferase	NULL				NULL		0	NULL	NULL	NULL	gw60_diabetes_50_11_2419_s_17	11679416	Glucose entry into this pathway is regulated by its first and rate-limiting enzyme, glutamine:fructose-6-phosphate amidotransferase (GFAT), which catalyzes the conversion of fructose-6-phosphate (F-6-P) and glutamine into glucosamine-6-phosphate (GlcN-6-P) and glutamate.	transcription
51659	2	334841	5	NULL	NULL	0	NULL	GFAT	NULL		is a type of	NULL				rate-limiting enzyme	NULL				NULL		0	NULL	NULL	NULL	gw60_diabetes_50_11_2419_s_17	11679416	Glucose entry into this pathway is regulated by its first and rate-limiting enzyme, glutamine:fructose-6-phosphate amidotransferase (GFAT), which catalyzes the conversion of fructose-6-phosphate (F-6-P) and glutamine into glucosamine-6-phosphate (GlcN-6-P) and glutamate.	transcription
51660	3	334841	5	NULL	NULL	0	NULL	F-6-P	NULL		is	NULL				fructose-6-phosphate	NULL				NULL		0	NULL	NULL	NULL	gw60_diabetes_50_11_2419_s_17	11679416	Glucose entry into this pathway is regulated by its first and rate-limiting enzyme, glutamine:fructose-6-phosphate amidotransferase (GFAT), which catalyzes the conversion of fructose-6-phosphate (F-6-P) and glutamine into glucosamine-6-phosphate (GlcN-6-P) and glutamate.	transcription
51661	4	334841	5	NULL	NULL	0	NULL	F-6-P	NULL		is converted to	NULL				GlcN-6-P	NULL				NULL		0	NULL	NULL	NULL	gw60_diabetes_50_11_2419_s_17	11679416	Glucose entry into this pathway is regulated by its first and rate-limiting enzyme, glutamine:fructose-6-phosphate amidotransferase (GFAT), which catalyzes the conversion of fructose-6-phosphate (F-6-P) and glutamine into glucosamine-6-phosphate (GlcN-6-P) and glutamate.	transcription
51662	5	334841	5	NULL	NULL	0	NULL	GlcN-6-P	NULL		is	NULL				glucosamine-6-phosphate	NULL				NULL		0	NULL	NULL	NULL	gw60_diabetes_50_11_2419_s_17	11679416	Glucose entry into this pathway is regulated by its first and rate-limiting enzyme, glutamine:fructose-6-phosphate amidotransferase (GFAT), which catalyzes the conversion of fructose-6-phosphate (F-6-P) and glutamine into glucosamine-6-phosphate (GlcN-6-P) and glutamate.	transcription
51663	6	334841	5	NULL	NULL	0	NULL	glutamine	NULL		is converted to	NULL				glutamate	NULL				NULL		0	NULL	NULL	NULL	gw60_diabetes_50_11_2419_s_17	11679416	Glucose entry into this pathway is regulated by its first and rate-limiting enzyme, glutamine:fructose-6-phosphate amidotransferase (GFAT), which catalyzes the conversion of fructose-6-phosphate (F-6-P) and glutamine into glucosamine-6-phosphate (GlcN-6-P) and glutamate.	transcription
51664	7	334841	5	NULL	NULL	0	NULL	GFAT	NULL		catalyzes	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_diabetes_50_11_2419_s_17	11679416	Glucose entry into this pathway is regulated by its first and rate-limiting enzyme, glutamine:fructose-6-phosphate amidotransferase (GFAT), which catalyzes the conversion of fructose-6-phosphate (F-6-P) and glutamine into glucosamine-6-phosphate (GlcN-6-P) and glutamate.	transcription
51665	8	334841	5	NULL	NULL	0	NULL	GFAT	NULL		catalyzes	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw60_diabetes_50_11_2419_s_17	11679416	Glucose entry into this pathway is regulated by its first and rate-limiting enzyme, glutamine:fructose-6-phosphate amidotransferase (GFAT), which catalyzes the conversion of fructose-6-phosphate (F-6-P) and glutamine into glucosamine-6-phosphate (GlcN-6-P) and glutamate.	transcription
52131	1	334841	6	NULL	NULL	0	NULL	fructose-6-phosphate	NULL		is converted to	NULL				glucosamine-6-phosphate	NULL				NULL		0	NULL	NULL	NULL	gw60_diabetes_50_11_2419_s_17	11679416	Glucose entry into this pathway is regulated by its first and rate-limiting enzyme, glutamine:fructose-6-phosphate amidotransferase (GFAT), which catalyzes the conversion of fructose-6-phosphate (F-6-P) and glutamine into glucosamine-6-phosphate (GlcN-6-P) and glutamate.	transcription
52132	2	334841	6	NULL	NULL	0	NULL	glucosamine-6-phosphate	NULL		is	NULL				GlcN-6-P	NULL				NULL		0	NULL	NULL	NULL	gw60_diabetes_50_11_2419_s_17	11679416	Glucose entry into this pathway is regulated by its first and rate-limiting enzyme, glutamine:fructose-6-phosphate amidotransferase (GFAT), which catalyzes the conversion of fructose-6-phosphate (F-6-P) and glutamine into glucosamine-6-phosphate (GlcN-6-P) and glutamate.	transcription
52133	3	334841	6	NULL	NULL	0	NULL	glutamine	NULL		is converted to	NULL				glutamate	NULL				NULL		0	NULL	NULL	NULL	gw60_diabetes_50_11_2419_s_17	11679416	Glucose entry into this pathway is regulated by its first and rate-limiting enzyme, glutamine:fructose-6-phosphate amidotransferase (GFAT), which catalyzes the conversion of fructose-6-phosphate (F-6-P) and glutamine into glucosamine-6-phosphate (GlcN-6-P) and glutamate.	transcription
52134	4	334841	6	NULL	NULL	0	NULL	F-6-P	NULL		is	NULL				fructose-6-phosphate	NULL				NULL		0	NULL	NULL	NULL	gw60_diabetes_50_11_2419_s_17	11679416	Glucose entry into this pathway is regulated by its first and rate-limiting enzyme, glutamine:fructose-6-phosphate amidotransferase (GFAT), which catalyzes the conversion of fructose-6-phosphate (F-6-P) and glutamine into glucosamine-6-phosphate (GlcN-6-P) and glutamate.	transcription
52135	5	334841	6	NULL	NULL	0	NULL	GFAT	NULL		catalyzes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_diabetes_50_11_2419_s_17	11679416	Glucose entry into this pathway is regulated by its first and rate-limiting enzyme, glutamine:fructose-6-phosphate amidotransferase (GFAT), which catalyzes the conversion of fructose-6-phosphate (F-6-P) and glutamine into glucosamine-6-phosphate (GlcN-6-P) and glutamate.	transcription
52136	6	334841	6	NULL	NULL	0	NULL	GFAT	NULL		catalyzes	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_diabetes_50_11_2419_s_17	11679416	Glucose entry into this pathway is regulated by its first and rate-limiting enzyme, glutamine:fructose-6-phosphate amidotransferase (GFAT), which catalyzes the conversion of fructose-6-phosphate (F-6-P) and glutamine into glucosamine-6-phosphate (GlcN-6-P) and glutamate.	transcription
52137	7	334841	6	NULL	NULL	0	NULL	GFAT	NULL		is	NULL				glutamine:fructose-6-phosphate amidotransferase	NULL				NULL		0	NULL	NULL	NULL	gw60_diabetes_50_11_2419_s_17	11679416	Glucose entry into this pathway is regulated by its first and rate-limiting enzyme, glutamine:fructose-6-phosphate amidotransferase (GFAT), which catalyzes the conversion of fructose-6-phosphate (F-6-P) and glutamine into glucosamine-6-phosphate (GlcN-6-P) and glutamate.	transcription
51666	1	334842	5	NULL	NULL	0	NULL	glutamine:fructose-6-phosphate amidotransferase	NULL		is a type of	NULL				rate-limiting enzyme in hexosamine biosynthetic pathway 	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_311_2_610_s_138	15240824	The availability of glucose and the rate-limiting enzyme glutamine:fructose-6-phosphate amidotransferase of the hexosamine biosynthetic pathway contribute to the regulation of cellular metabolism by glucose (Singh et al., 2001 ).	transcription
51667	2	334842	5	NULL	NULL	0	NULL	glucose	NULL		plays a role in	NULL				cellular metabolism	NULL				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_311_2_610_s_138	15240824	The availability of glucose and the rate-limiting enzyme glutamine:fructose-6-phosphate amidotransferase of the hexosamine biosynthetic pathway contribute to the regulation of cellular metabolism by glucose (Singh et al., 2001 ).	transcription
51668	3	334842	5	NULL	NULL	0	NULL	glutamine:fructose-6-phosphate amidotransferase	NULL		regulates	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_311_2_610_s_138	15240824	The availability of glucose and the rate-limiting enzyme glutamine:fructose-6-phosphate amidotransferase of the hexosamine biosynthetic pathway contribute to the regulation of cellular metabolism by glucose (Singh et al., 2001 ).	transcription
51669	4	334842	5	NULL	NULL	0	NULL	glucose	NULL	availability of	regulates	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_311_2_610_s_138	15240824	The availability of glucose and the rate-limiting enzyme glutamine:fructose-6-phosphate amidotransferase of the hexosamine biosynthetic pathway contribute to the regulation of cellular metabolism by glucose (Singh et al., 2001 ).	transcription
52419	1	334842	6	NULL	NULL	0	NULL	glucose	NULL		regulates	NULL				cell metabolism	NULL				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_311_2_610_s_138	15240824	The availability of glucose and the rate-limiting enzyme glutamine:fructose-6-phosphate amidotransferase of the hexosamine biosynthetic pathway contribute to the regulation of cellular metabolism by glucose (Singh et al., 2001 ).	transcription
52468	2	334842	6	NULL	NULL	0	NULL	glucose	NULL	availability of 	contributes to	NULL				statement 1	NULL	regulation of 			NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_311_2_610_s_138	15240824	The availability of glucose and the rate-limiting enzyme glutamine:fructose-6-phosphate amidotransferase of the hexosamine biosynthetic pathway contribute to the regulation of cellular metabolism by glucose (Singh et al., 2001 ).	transcription
52469	3	334842	6	NULL	NULL	0	NULL	 glutamine:fructose-6-phosphate amidotransferase	NULL	availability of 	contributes to	NULL				statement 1	NULL	regulation of 			NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_311_2_610_s_138	15240824	The availability of glucose and the rate-limiting enzyme glutamine:fructose-6-phosphate amidotransferase of the hexosamine biosynthetic pathway contribute to the regulation of cellular metabolism by glucose (Singh et al., 2001 ).	transcription
51670	1	334843	5	NULL	NULL	0	NULL	hexokinase	NULL		is a type of	NULL				enzyme	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1626_1_57_s_102	12697330	The enzyme hexokinase phosphorylates both glucose and fructose to give respective  hexose-6-phosphate, while glucose-6-phosphate isomerase catalyzes the isomerization  of fructose-6-phosphate from/to glucose-6-phosphate.	transcription
51671	2	334843	5	NULL	NULL	0	NULL	hexokinase	NULL		phosphorylates	NULL				glucose	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1626_1_57_s_102	12697330	The enzyme hexokinase phosphorylates both glucose and fructose to give respective  hexose-6-phosphate, while glucose-6-phosphate isomerase catalyzes the isomerization  of fructose-6-phosphate from/to glucose-6-phosphate.	transcription
51672	3	334843	5	NULL	NULL	0	NULL	statement 2	NULL		forms	NULL				glucose-6-phosphate	NULL				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1626_1_57_s_102	12697330	The enzyme hexokinase phosphorylates both glucose and fructose to give respective  hexose-6-phosphate, while glucose-6-phosphate isomerase catalyzes the isomerization  of fructose-6-phosphate from/to glucose-6-phosphate.	transcription
51673	4	334843	5	NULL	NULL	0	NULL	hexokinase	NULL		phosphorylates	NULL				fructose	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1626_1_57_s_102	12697330	The enzyme hexokinase phosphorylates both glucose and fructose to give respective  hexose-6-phosphate, while glucose-6-phosphate isomerase catalyzes the isomerization  of fructose-6-phosphate from/to glucose-6-phosphate.	transcription
51674	5	334843	5	NULL	NULL	0	NULL	statement 4	NULL		forms	NULL				fructose-6-phosphate	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1626_1_57_s_102	12697330	The enzyme hexokinase phosphorylates both glucose and fructose to give respective  hexose-6-phosphate, while glucose-6-phosphate isomerase catalyzes the isomerization  of fructose-6-phosphate from/to glucose-6-phosphate.	transcription
51675	6	334843	5	NULL	NULL	0	NULL	fructose-6-phosphate	NULL		is isomerized to	NULL				glucose-6-phosphate	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1626_1_57_s_102	12697330	The enzyme hexokinase phosphorylates both glucose and fructose to give respective  hexose-6-phosphate, while glucose-6-phosphate isomerase catalyzes the isomerization  of fructose-6-phosphate from/to glucose-6-phosphate.	transcription
51676	7	334843	5	NULL	NULL	0	NULL	fructose-6-phosphate	NULL		is isomerized from	NULL				glucose-6-phosphate	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1626_1_57_s_102	12697330	The enzyme hexokinase phosphorylates both glucose and fructose to give respective  hexose-6-phosphate, while glucose-6-phosphate isomerase catalyzes the isomerization  of fructose-6-phosphate from/to glucose-6-phosphate.	transcription
51677	8	334843	5	NULL	NULL	0	NULL	glucose-6-phosphate isomerase	NULL		catalyzes	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1626_1_57_s_102	12697330	The enzyme hexokinase phosphorylates both glucose and fructose to give respective  hexose-6-phosphate, while glucose-6-phosphate isomerase catalyzes the isomerization  of fructose-6-phosphate from/to glucose-6-phosphate.	transcription
51678	9	334843	5	NULL	NULL	0	NULL	glucose-6-phosphate isomerase	NULL		catalyzes	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1626_1_57_s_102	12697330	The enzyme hexokinase phosphorylates both glucose and fructose to give respective  hexose-6-phosphate, while glucose-6-phosphate isomerase catalyzes the isomerization  of fructose-6-phosphate from/to glucose-6-phosphate.	transcription
52470	1	334843	6	NULL	NULL	0	NULL	glucose	NULL		is phosphorylated to	NULL				glucose-6-phosphate	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1626_1_57_s_102	12697330	The enzyme hexokinase phosphorylates both glucose and fructose to give respective  hexose-6-phosphate, while glucose-6-phosphate isomerase catalyzes the isomerization  of fructose-6-phosphate from/to glucose-6-phosphate.	transcription
52471	2	334843	6	NULL	NULL	0	NULL	fructose	NULL		is phosphorylated to	NULL				fructose-6-phosphate	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1626_1_57_s_102	12697330	The enzyme hexokinase phosphorylates both glucose and fructose to give respective  hexose-6-phosphate, while glucose-6-phosphate isomerase catalyzes the isomerization  of fructose-6-phosphate from/to glucose-6-phosphate.	transcription
52472	3	334843	6	NULL	NULL	0	NULL	hexokinase	NULL		catalyzes	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1626_1_57_s_102	12697330	The enzyme hexokinase phosphorylates both glucose and fructose to give respective  hexose-6-phosphate, while glucose-6-phosphate isomerase catalyzes the isomerization  of fructose-6-phosphate from/to glucose-6-phosphate.	transcription
52473	4	334843	6	NULL	NULL	0	NULL	hexokinase	NULL		catalyzes	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1626_1_57_s_102	12697330	The enzyme hexokinase phosphorylates both glucose and fructose to give respective  hexose-6-phosphate, while glucose-6-phosphate isomerase catalyzes the isomerization  of fructose-6-phosphate from/to glucose-6-phosphate.	transcription
52474	5	334843	6	NULL	NULL	0	NULL	fructose-6-phosphate	NULL		is isomerized to	NULL				glucose-6-phosphate	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1626_1_57_s_102	12697330	The enzyme hexokinase phosphorylates both glucose and fructose to give respective  hexose-6-phosphate, while glucose-6-phosphate isomerase catalyzes the isomerization  of fructose-6-phosphate from/to glucose-6-phosphate.	transcription
52475	6	334843	6	NULL	NULL	0	NULL	glucose-6-phosphate isomerase 	NULL		catalyzes	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1626_1_57_s_102	12697330	The enzyme hexokinase phosphorylates both glucose and fructose to give respective  hexose-6-phosphate, while glucose-6-phosphate isomerase catalyzes the isomerization  of fructose-6-phosphate from/to glucose-6-phosphate.	transcription
51679	1	334844	5	NULL	NULL	0	NULL	hexosamine	NULL		induces	NULL				insulin resistance	NULL				NULL	transgenic mice overexpressing glutamine: fructose-6-phosphate amidotransferase	NULL	NULL	NULL	NULL	gw60_gene_261_2_329_s_219	11167021	Mechanism of hexosamine-induced insulin resistance in transgenic mice overexpressing glutamine: fructose-6-phosphate amidotransferase: decreased glucose transporter GLUT4 translocation and reversal by treatment with thiazolidinedione.	transcription
52476	1	334844	6	NULL	NULL	0	NULL	hexosamine	NULL		induces	NULL				insulin	NULL	resistance to			NULL	transgenic mice overexpressing glutamine: fructose-6-phosphate amidotransferase	0	NULL	NULL	NULL	gw60_gene_261_2_329_s_219	11167021	Mechanism of hexosamine-induced insulin resistance in transgenic mice overexpressing glutamine: fructose-6-phosphate amidotransferase: decreased glucose transporter GLUT4 translocation and reversal by treatment with thiazolidinedione.	transcription
52477	2	334844	6	NULL	NULL	0	NULL	GLUT4	NULL		is a type of	NULL				glucose transporter	NULL				NULL		0	NULL	NULL	NULL	gw60_gene_261_2_329_s_219	11167021	Mechanism of hexosamine-induced insulin resistance in transgenic mice overexpressing glutamine: fructose-6-phosphate amidotransferase: decreased glucose transporter GLUT4 translocation and reversal by treatment with thiazolidinedione.	transcription
51680	1	334845	5	NULL	NULL	0	NULL	regulatory protein	NULL		bind	NULL				fructose-6-phosphate	NULL				NULL		0	NULL	NULL	NULL	gw60_diabetes_50_6_1263_s_16	11375325	lucokinase    activity is acutely regulated by interaction with a regulatory protein ( 1) that binds to fructose-6-phosphate (P) and allosterically inhibits glucokinase by lowering the enzyme s affinity for glucose.	transcription
51681	4	334845	5	NULL	NULL	0	NULL	statement 3	NULL		inhibit	NULL	allosterically			glucokinase	NULL				NULL		NULL	NULL	NULL	NULL	gw60_diabetes_50_6_1263_s_16	11375325	lucokinase    activity is acutely regulated by interaction with a regulatory protein ( 1) that binds to fructose-6-phosphate (P) and allosterically inhibits glucokinase by lowering the enzyme s affinity for glucose.	transcription
51682	2	334845	5	NULL	NULL	0	NULL	glucokinase	NULL		has affinity for	NULL				glucose	NULL				NULL		NULL	NULL	NULL	NULL	gw60_diabetes_50_6_1263_s_16	11375325	lucokinase    activity is acutely regulated by interaction with a regulatory protein ( 1) that binds to fructose-6-phosphate (P) and allosterically inhibits glucokinase by lowering the enzyme s affinity for glucose.	transcription
51683	3	334845	5	NULL	NULL	0	NULL	statement 1	NULL		lowers	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_diabetes_50_6_1263_s_16	11375325	lucokinase    activity is acutely regulated by interaction with a regulatory protein ( 1) that binds to fructose-6-phosphate (P) and allosterically inhibits glucokinase by lowering the enzyme s affinity for glucose.	transcription
52478	1	334845	6	NULL	NULL	0	NULL	regulatory protein	NULL		bind	NULL				fructose-6-phosphate	NULL				NULL		0	NULL	NULL	NULL	gw60_diabetes_50_6_1263_s_16	11375325	lucokinase    activity is acutely regulated by interaction with a regulatory protein ( 1) that binds to fructose-6-phosphate (P) and allosterically inhibits glucokinase by lowering the enzyme s affinity for glucose.	transcription
52479	2	334845	6	NULL	NULL	0	NULL	regulatory protein	NULL		inhibits	NULL	allosterically			glucokinase	NULL				NULL		0	NULL	NULL	NULL	gw60_diabetes_50_6_1263_s_16	11375325	lucokinase    activity is acutely regulated by interaction with a regulatory protein ( 1) that binds to fructose-6-phosphate (P) and allosterically inhibits glucokinase by lowering the enzyme s affinity for glucose.	transcription
52480	3	334845	6	NULL	NULL	0	NULL	lucokinase	NULL		interacts with	NULL				regulatory protein	NULL				NULL		0	NULL	NULL	NULL	gw60_diabetes_50_6_1263_s_16	11375325	lucokinase    activity is acutely regulated by interaction with a regulatory protein ( 1) that binds to fructose-6-phosphate (P) and allosterically inhibits glucokinase by lowering the enzyme s affinity for glucose.	transcription
52481	4	334845	6	NULL	NULL	0	NULL	statement 3	NULL		regulates	NULL				lucokinase	NULL	activity of 			NULL		0	NULL	NULL	NULL	gw60_diabetes_50_6_1263_s_16	11375325	lucokinase    activity is acutely regulated by interaction with a regulatory protein ( 1) that binds to fructose-6-phosphate (P) and allosterically inhibits glucokinase by lowering the enzyme s affinity for glucose.	transcription
51684	1	334846	5	NULL	NULL	0	NULL	glucose	NULL		induce	NULL					NULL	activation of		GlRE	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_7	14757763	The high glucose-induced activation of the GlRE is mediated by the HBP; increased flux through the HBP induced by high glucose concentrations, by glutamine, or by overexpression of the rate-limiting enzyme glutamine:fructose-6-phosphate aminotransferase (GFAT) particularly activated USF-2 expression.	transcription
51685	2	334846	5	NULL	NULL	0	NULL	HBP	NULL		mediate	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_7	14757763	The high glucose-induced activation of the GlRE is mediated by the HBP; increased flux through the HBP induced by high glucose concentrations, by glutamine, or by overexpression of the rate-limiting enzyme glutamine:fructose-6-phosphate aminotransferase (GFAT) particularly activated USF-2 expression.	transcription
51687	3	334846	5	NULL	NULL	0	NULL	GFAT	NULL		is	NULL				glutamine:fructose-6-phosphate aminotransferase	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_7	14757763	The high glucose-induced activation of the GlRE is mediated by the HBP; increased flux through the HBP induced by high glucose concentrations, by glutamine, or by overexpression of the rate-limiting enzyme glutamine:fructose-6-phosphate aminotransferase (GFAT) particularly activated USF-2 expression.	transcription
51688	4	334846	5	NULL	NULL	0	NULL	glucose	NULL	high concentration of	induce	NULL				HBP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_7	14757763	The high glucose-induced activation of the GlRE is mediated by the HBP; increased flux through the HBP induced by high glucose concentrations, by glutamine, or by overexpression of the rate-limiting enzyme glutamine:fructose-6-phosphate aminotransferase (GFAT) particularly activated USF-2 expression.	transcription
51689	5	334846	5	NULL	NULL	0	NULL	statement 4	NULL		increases	NULL				flux	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_7	14757763	The high glucose-induced activation of the GlRE is mediated by the HBP; increased flux through the HBP induced by high glucose concentrations, by glutamine, or by overexpression of the rate-limiting enzyme glutamine:fructose-6-phosphate aminotransferase (GFAT) particularly activated USF-2 expression.	transcription
51690	6	334846	5	NULL	NULL	0	NULL	statement 5	NULL		activates	NULL				USF-2	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_7	14757763	The high glucose-induced activation of the GlRE is mediated by the HBP; increased flux through the HBP induced by high glucose concentrations, by glutamine, or by overexpression of the rate-limiting enzyme glutamine:fructose-6-phosphate aminotransferase (GFAT) particularly activated USF-2 expression.	transcription
51691	7	334846	5	NULL	NULL	0	NULL	glutamine	NULL		induce	NULL				HBP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_7	14757763	The high glucose-induced activation of the GlRE is mediated by the HBP; increased flux through the HBP induced by high glucose concentrations, by glutamine, or by overexpression of the rate-limiting enzyme glutamine:fructose-6-phosphate aminotransferase (GFAT) particularly activated USF-2 expression.	transcription
51692	8	334846	5	NULL	NULL	0	NULL	statement 7	NULL		increases	NULL				flux	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_7	14757763	The high glucose-induced activation of the GlRE is mediated by the HBP; increased flux through the HBP induced by high glucose concentrations, by glutamine, or by overexpression of the rate-limiting enzyme glutamine:fructose-6-phosphate aminotransferase (GFAT) particularly activated USF-2 expression.	transcription
51693	9	334846	5	NULL	NULL	0	NULL	statement 8	NULL		activates	NULL				USF-2	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_7	14757763	The high glucose-induced activation of the GlRE is mediated by the HBP; increased flux through the HBP induced by high glucose concentrations, by glutamine, or by overexpression of the rate-limiting enzyme glutamine:fructose-6-phosphate aminotransferase (GFAT) particularly activated USF-2 expression.	transcription
51694	10	334846	5	NULL	NULL	0	NULL	GFAT	NULL	overexpression of	induce	NULL				HBP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_7	14757763	The high glucose-induced activation of the GlRE is mediated by the HBP; increased flux through the HBP induced by high glucose concentrations, by glutamine, or by overexpression of the rate-limiting enzyme glutamine:fructose-6-phosphate aminotransferase (GFAT) particularly activated USF-2 expression.	transcription
51695	11	334846	5	NULL	NULL	0	NULL	statement 10	NULL		increases	NULL				flux	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_7	14757763	The high glucose-induced activation of the GlRE is mediated by the HBP; increased flux through the HBP induced by high glucose concentrations, by glutamine, or by overexpression of the rate-limiting enzyme glutamine:fructose-6-phosphate aminotransferase (GFAT) particularly activated USF-2 expression.	transcription
51696	12	334846	5	NULL	NULL	0	NULL	statement 11	NULL		activates	NULL				USF-2	NULL	expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_7	14757763	The high glucose-induced activation of the GlRE is mediated by the HBP; increased flux through the HBP induced by high glucose concentrations, by glutamine, or by overexpression of the rate-limiting enzyme glutamine:fructose-6-phosphate aminotransferase (GFAT) particularly activated USF-2 expression.	transcription
52482	1	334846	6	NULL	NULL	0	NULL	glucose	NULL		induces	NULL				GIRE	NULL	activation of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_7	14757763	The high glucose-induced activation of the GlRE is mediated by the HBP; increased flux through the HBP induced by high glucose concentrations, by glutamine, or by overexpression of the rate-limiting enzyme glutamine:fructose-6-phosphate aminotransferase (GFAT) particularly activated USF-2 expression.	transcription
52524	2	334846	6	NULL	NULL	0	NULL	HBP	NULL		mediates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_7	14757763	The high glucose-induced activation of the GlRE is mediated by the HBP; increased flux through the HBP induced by high glucose concentrations, by glutamine, or by overexpression of the rate-limiting enzyme glutamine:fructose-6-phosphate aminotransferase (GFAT) particularly activated USF-2 expression.	transcription
52525	3	334846	6	NULL	NULL	0	NULL	glucose	NULL	high concentration of 	induces	NULL				HBP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_7	14757763	The high glucose-induced activation of the GlRE is mediated by the HBP; increased flux through the HBP induced by high glucose concentrations, by glutamine, or by overexpression of the rate-limiting enzyme glutamine:fructose-6-phosphate aminotransferase (GFAT) particularly activated USF-2 expression.	transcription
52526	4	334846	6	NULL	NULL	0	NULL	statement 3	NULL		increases	NULL				flux	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_7	14757763	The high glucose-induced activation of the GlRE is mediated by the HBP; increased flux through the HBP induced by high glucose concentrations, by glutamine, or by overexpression of the rate-limiting enzyme glutamine:fructose-6-phosphate aminotransferase (GFAT) particularly activated USF-2 expression.	transcription
52527	5	334846	6	NULL	NULL	0	NULL	statement 4	NULL		activates	NULL				USF-2	NULL	expression of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_7	14757763	The high glucose-induced activation of the GlRE is mediated by the HBP; increased flux through the HBP induced by high glucose concentrations, by glutamine, or by overexpression of the rate-limiting enzyme glutamine:fructose-6-phosphate aminotransferase (GFAT) particularly activated USF-2 expression.	transcription
52528	6	334846	6	NULL	NULL	0	NULL	GFAT	NULL	overexpression of	activates	NULL				USF-2	NULL	expression of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_7	14757763	The high glucose-induced activation of the GlRE is mediated by the HBP; increased flux through the HBP induced by high glucose concentrations, by glutamine, or by overexpression of the rate-limiting enzyme glutamine:fructose-6-phosphate aminotransferase (GFAT) particularly activated USF-2 expression.	transcription
52529	7	334846	6	NULL	NULL	0	NULL	GFAT	NULL		is	NULL				glutamine:fructose-6-phosphate aminotransferase	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_7	14757763	The high glucose-induced activation of the GlRE is mediated by the HBP; increased flux through the HBP induced by high glucose concentrations, by glutamine, or by overexpression of the rate-limiting enzyme glutamine:fructose-6-phosphate aminotransferase (GFAT) particularly activated USF-2 expression.	transcription
51697	1	334847	5	NULL	NULL	0	NULL	G3P & glucose	NULL	addition of	reduces	NULL				beta-galactosidase	NULL	activity of			NULL		0	NULL	NULL	NULL	abs-batch0680-0699_fems-microbiol-lett_162_1_9595668_s_5	9595668	When G3P and glucose, glucose-6-phosphate or fructose-6-phosphate  were added, beta-galactosidase activity was reduced showing that GlpP  mediates catabolite repression of transcription from the glpD leader in  the absence of any other B. subtilis protein.	transcription
51698	2	334847	5	NULL	NULL	0	NULL	G3P & glucose-6-phosphate	NULL	addition of	reduces	NULL				beta-galactosidase	NULL	activity of			NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_fems-microbiol-lett_162_1_9595668_s_5	9595668	When G3P and glucose, glucose-6-phosphate or fructose-6-phosphate  were added, beta-galactosidase activity was reduced showing that GlpP  mediates catabolite repression of transcription from the glpD leader in  the absence of any other B. subtilis protein.	transcription
51699	3	334847	5	NULL	NULL	0	NULL	G3P & fructose-6-phosphate	NULL	addition of	reduces	NULL				beta-galactosidase	NULL	activity of			NULL		0	NULL	NULL	NULL	abs-batch0680-0699_fems-microbiol-lett_162_1_9595668_s_5	9595668	When G3P and glucose, glucose-6-phosphate or fructose-6-phosphate  were added, beta-galactosidase activity was reduced showing that GlpP  mediates catabolite repression of transcription from the glpD leader in  the absence of any other B. subtilis protein.	transcription
51700	4	334847	5	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_fems-microbiol-lett_162_1_9595668_s_5	9595668	When G3P and glucose, glucose-6-phosphate or fructose-6-phosphate  were added, beta-galactosidase activity was reduced showing that GlpP  mediates catabolite repression of transcription from the glpD leader in  the absence of any other B. subtilis protein.	transcription
51701	5	334847	5	NULL	NULL	0	NULL	statement 2	NULL		is an alternative to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_fems-microbiol-lett_162_1_9595668_s_5	9595668	When G3P and glucose, glucose-6-phosphate or fructose-6-phosphate  were added, beta-galactosidase activity was reduced showing that GlpP  mediates catabolite repression of transcription from the glpD leader in  the absence of any other B. subtilis protein.	transcription
51702	6	334847	5	NULL	NULL	0	NULL	GlpP	NULL		mediates	NULL				glpD	NULL	catabolite repression of;;transcription of		leader	NULL		NULL	NULL	NULL	NULL	abs-batch0680-0699_fems-microbiol-lett_162_1_9595668_s_5	9595668	When G3P and glucose, glucose-6-phosphate or fructose-6-phosphate  were added, beta-galactosidase activity was reduced showing that GlpP  mediates catabolite repression of transcription from the glpD leader in  the absence of any other B. subtilis protein.	transcription
51703	7	334847	5	NULL	NULL	0	NULL	statement 6	NULL		in the absence of	NULL				protein	NULL	B. subtilis			NULL		0	NULL	NULL	NULL	abs-batch0680-0699_fems-microbiol-lett_162_1_9595668_s_5	9595668	When G3P and glucose, glucose-6-phosphate or fructose-6-phosphate  were added, beta-galactosidase activity was reduced showing that GlpP  mediates catabolite repression of transcription from the glpD leader in  the absence of any other B. subtilis protein.	transcription
52530	1	334847	6	NULL	NULL	0	NULL	GlpP	NULL		mediates	NULL				transcription	NULL	catabolite repression of 			NULL		0	NULL	NULL	NULL	abs-batch0680-0699_fems-microbiol-lett_162_1_9595668_s_5	9595668	When G3P and glucose, glucose-6-phosphate or fructose-6-phosphate  were added, beta-galactosidase activity was reduced showing that GlpP  mediates catabolite repression of transcription from the glpD leader in  the absence of any other B. subtilis protein.	transcription
51704	1	334848	5	NULL	NULL	0	NULL	GFAT	NULL		is	NULL				glutamine:fructose-6-phosphate amidotransferase	NULL				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_1_93_s_91	16380481	The ability of 20 mumol/l azaserine, a potent inhibitor of GFAT (glutamine:fructose-6-phosphate amidotransferase), to attenuate glucose, but not glucosamine-induced ER stress, suggests that elevated concentrations of glucose cause ER stress through a glucosamine intermediate ( Fig. 1 B).	transcription
51705	2	334848	5	NULL	NULL	0	NULL	azaserine	NULL		is an inhibitor of	NULL	potent			GFAT	NULL				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_1_93_s_91	16380481	The ability of 20 mumol/l azaserine, a potent inhibitor of GFAT (glutamine:fructose-6-phosphate amidotransferase), to attenuate glucose, but not glucosamine-induced ER stress, suggests that elevated concentrations of glucose cause ER stress through a glucosamine intermediate ( Fig. 1 B).	transcription
51706	3	334848	5	NULL	NULL	0	NULL	azaserine	NULL		attenuate	NULL				glucose	NULL				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_1_93_s_91	16380481	The ability of 20 mumol/l azaserine, a potent inhibitor of GFAT (glutamine:fructose-6-phosphate amidotransferase), to attenuate glucose, but not glucosamine-induced ER stress, suggests that elevated concentrations of glucose cause ER stress through a glucosamine intermediate ( Fig. 1 B).	transcription
51707	4	334848	5	NULL	NULL	0	NULL	ER stress	NULL		is induced by	NULL				glucosamine	NULL				NULL		NULL	NULL	NULL	NULL	gw70_diabetes_55_1_93_s_91	16380481	The ability of 20 mumol/l azaserine, a potent inhibitor of GFAT (glutamine:fructose-6-phosphate amidotransferase), to attenuate glucose, but not glucosamine-induced ER stress, suggests that elevated concentrations of glucose cause ER stress through a glucosamine intermediate ( Fig. 1 B).	transcription
51708	5	334848	5	NULL	NULL	0	NULL	azaserine	NULL		does not attenuate	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_1_93_s_91	16380481	The ability of 20 mumol/l azaserine, a potent inhibitor of GFAT (glutamine:fructose-6-phosphate amidotransferase), to attenuate glucose, but not glucosamine-induced ER stress, suggests that elevated concentrations of glucose cause ER stress through a glucosamine intermediate ( Fig. 1 B).	transcription
51709	6	334848	5	NULL	NULL	0	NULL	glucose	NULL	elevated concentrations	causes	NULL				ER stress	NULL				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_1_93_s_91	16380481	The ability of 20 mumol/l azaserine, a potent inhibitor of GFAT (glutamine:fructose-6-phosphate amidotransferase), to attenuate glucose, but not glucosamine-induced ER stress, suggests that elevated concentrations of glucose cause ER stress through a glucosamine intermediate ( Fig. 1 B).	transcription
51710	7	334848	5	NULL	NULL	0	NULL	statement 6	NULL		occurs through	NULL				glucosamine intermediate	NULL				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_1_93_s_91	16380481	The ability of 20 mumol/l azaserine, a potent inhibitor of GFAT (glutamine:fructose-6-phosphate amidotransferase), to attenuate glucose, but not glucosamine-induced ER stress, suggests that elevated concentrations of glucose cause ER stress through a glucosamine intermediate ( Fig. 1 B).	transcription
52531	1	334848	6	NULL	NULL	0	NULL	glucose	NULL	elevated concentrations of	cause	NULL				ER stress	NULL				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_1_93_s_91	16380481	The ability of 20 mumol/l azaserine, a potent inhibitor of GFAT (glutamine:fructose-6-phosphate amidotransferase), to attenuate glucose, but not glucosamine-induced ER stress, suggests that elevated concentrations of glucose cause ER stress through a glucosamine intermediate ( Fig. 1 B).	transcription
52532	2	334848	6	NULL	NULL	0	NULL	statement 1	NULL		occurs through	NULL				glucosamine intermediate	NULL				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_1_93_s_91	16380481	The ability of 20 mumol/l azaserine, a potent inhibitor of GFAT (glutamine:fructose-6-phosphate amidotransferase), to attenuate glucose, but not glucosamine-induced ER stress, suggests that elevated concentrations of glucose cause ER stress through a glucosamine intermediate ( Fig. 1 B).	transcription
52533	3	334848	6	NULL	NULL	0	NULL	azaserine	NULL		is a type of 	NULL				inhibitor of GFAT	NULL				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_1_93_s_91	16380481	The ability of 20 mumol/l azaserine, a potent inhibitor of GFAT (glutamine:fructose-6-phosphate amidotransferase), to attenuate glucose, but not glucosamine-induced ER stress, suggests that elevated concentrations of glucose cause ER stress through a glucosamine intermediate ( Fig. 1 B).	transcription
52534	4	334848	6	NULL	NULL	0	NULL	GFAT	NULL		is	NULL				glutamine:fructose-6-phosphate amidotransferase	NULL				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_1_93_s_91	16380481	The ability of 20 mumol/l azaserine, a potent inhibitor of GFAT (glutamine:fructose-6-phosphate amidotransferase), to attenuate glucose, but not glucosamine-induced ER stress, suggests that elevated concentrations of glucose cause ER stress through a glucosamine intermediate ( Fig. 1 B).	transcription
52535	5	334848	6	NULL	NULL	0	NULL	azaserine	NULL		attenuates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_1_93_s_91	16380481	The ability of 20 mumol/l azaserine, a potent inhibitor of GFAT (glutamine:fructose-6-phosphate amidotransferase), to attenuate glucose, but not glucosamine-induced ER stress, suggests that elevated concentrations of glucose cause ER stress through a glucosamine intermediate ( Fig. 1 B).	transcription
52536	6	334848	6	NULL	NULL	0	NULL	glucosamine	NULL		induces	NULL				ER stress	NULL				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_1_93_s_91	16380481	The ability of 20 mumol/l azaserine, a potent inhibitor of GFAT (glutamine:fructose-6-phosphate amidotransferase), to attenuate glucose, but not glucosamine-induced ER stress, suggests that elevated concentrations of glucose cause ER stress through a glucosamine intermediate ( Fig. 1 B).	transcription
52537	7	334848	6	NULL	NULL	0	NULL	azaserine	NULL		does not attenuate	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_1_93_s_91	16380481	The ability of 20 mumol/l azaserine, a potent inhibitor of GFAT (glutamine:fructose-6-phosphate amidotransferase), to attenuate glucose, but not glucosamine-induced ER stress, suggests that elevated concentrations of glucose cause ER stress through a glucosamine intermediate ( Fig. 1 B).	transcription
51711	1	334849	5	NULL	NULL	0	NULL	azaserine	NULL		is an inhibitor of	NULL				glutamine/fructose-6-phosphate amidotransferase	NULL				NULL		0	NULL	NULL	NULL	gw70_diabetes_53_4_890_s_193	15047603	To evaluate whether the hexosamine pathway could mediate the induction of FXR expression by D-glucose, rat hepatocytes were cultured with azaserine (5 mumol/l), an inhibitor of glutamine/fructose-6-phosphate amidotransferase, the rate-limiting enzyme in the conversion of glucose to glucosamine.	transcription
51712	2	334849	5	NULL	NULL	0	NULL	glucose	NULL		is converted to	NULL				glucosamine	NULL				NULL		0	NULL	NULL	NULL	gw70_diabetes_53_4_890_s_193	15047603	To evaluate whether the hexosamine pathway could mediate the induction of FXR expression by D-glucose, rat hepatocytes were cultured with azaserine (5 mumol/l), an inhibitor of glutamine/fructose-6-phosphate amidotransferase, the rate-limiting enzyme in the conversion of glucose to glucosamine.	transcription
51713	3	334849	5	NULL	NULL	0	NULL	FXR	NULL	expression of	is induced by	NULL				D-glucose	NULL				NULL	rat hepatocytes	NULL	NULL	NULL	NULL	gw70_diabetes_53_4_890_s_193	15047603	To evaluate whether the hexosamine pathway could mediate the induction of FXR expression by D-glucose, rat hepatocytes were cultured with azaserine (5 mumol/l), an inhibitor of glutamine/fructose-6-phosphate amidotransferase, the rate-limiting enzyme in the conversion of glucose to glucosamine.	transcription
52037	4	334849	5	NULL	NULL	0	NULL	hexosamine pathway	NULL		mediate	NULL	may			statement 3	NULL				NULL	rat hepatocytes	0	NULL	NULL	NULL	gw70_diabetes_53_4_890_s_193	15047603	To evaluate whether the hexosamine pathway could mediate the induction of FXR expression by D-glucose, rat hepatocytes were cultured with azaserine (5 mumol/l), an inhibitor of glutamine/fructose-6-phosphate amidotransferase, the rate-limiting enzyme in the conversion of glucose to glucosamine.	transcription
52538	1	334849	6	NULL	NULL	0	NULL	glucose	NULL		is converted to	NULL				glucosamine	NULL				NULL		0	NULL	NULL	NULL	gw70_diabetes_53_4_890_s_193	15047603	To evaluate whether the hexosamine pathway could mediate the induction of FXR expression by D-glucose, rat hepatocytes were cultured with azaserine (5 mumol/l), an inhibitor of glutamine/fructose-6-phosphate amidotransferase, the rate-limiting enzyme in the conversion of glucose to glucosamine.	transcription
52539	2	334849	6	NULL	NULL	0	NULL	glutamine/fructose-6-phosphate amidotransferase	NULL		catalyzes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_diabetes_53_4_890_s_193	15047603	To evaluate whether the hexosamine pathway could mediate the induction of FXR expression by D-glucose, rat hepatocytes were cultured with azaserine (5 mumol/l), an inhibitor of glutamine/fructose-6-phosphate amidotransferase, the rate-limiting enzyme in the conversion of glucose to glucosamine.	transcription
51714	1	334850	5	NULL	NULL	0	NULL	hexosamine	NULL		induce	NULL				insulin resistance	NULL				NULL	transgenic mice overexpressing glutamine:fructose-6-phosphate amidotransferase	0	NULL	NULL	NULL	gw60_diabetes_50_5_1093_s_411	11334413	Diabetes 45:1644 - 1654, 1996 [Abstract]    Cooksey RC, Hebert LF, Zhu JH, Wofford P, Garvey WT, McClain DA: Mechanism of hexosamine-induced insulin resistance in transgenic mice overexpressing glutamine:fructose-6-phosphate amidotransferase: decreased glucose transporter GLUT4 translocation and reversal by treatment with thiazolidinedione.	transcription
51715	2	334850	5	NULL	NULL	0	NULL	statement 1	NULL		decreases	NULL				GLUT4	NULL	translocation of			NULL		0	NULL	NULL	NULL	gw60_diabetes_50_5_1093_s_411	11334413	Diabetes 45:1644 - 1654, 1996 [Abstract]    Cooksey RC, Hebert LF, Zhu JH, Wofford P, Garvey WT, McClain DA: Mechanism of hexosamine-induced insulin resistance in transgenic mice overexpressing glutamine:fructose-6-phosphate amidotransferase: decreased glucose transporter GLUT4 translocation and reversal by treatment with thiazolidinedione.	transcription
51716	3	334850	5	NULL	NULL	0	NULL	GLUT4	NULL		is a type of	NULL				glucose transporter	NULL				NULL		0	NULL	NULL	NULL	gw60_diabetes_50_5_1093_s_411	11334413	Diabetes 45:1644 - 1654, 1996 [Abstract]    Cooksey RC, Hebert LF, Zhu JH, Wofford P, Garvey WT, McClain DA: Mechanism of hexosamine-induced insulin resistance in transgenic mice overexpressing glutamine:fructose-6-phosphate amidotransferase: decreased glucose transporter GLUT4 translocation and reversal by treatment with thiazolidinedione.	transcription
51717	4	334850	5	NULL	NULL	0	NULL	thiazolidinedione	NULL	treatment	reverse	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_diabetes_50_5_1093_s_411	11334413	Diabetes 45:1644 - 1654, 1996 [Abstract]    Cooksey RC, Hebert LF, Zhu JH, Wofford P, Garvey WT, McClain DA: Mechanism of hexosamine-induced insulin resistance in transgenic mice overexpressing glutamine:fructose-6-phosphate amidotransferase: decreased glucose transporter GLUT4 translocation and reversal by treatment with thiazolidinedione.	transcription
52540	1	334850	6	NULL	NULL	0	NULL	hexosamine	NULL		induces	NULL				insulin	NULL	resistance to			NULL	transgenic mice overexpressing glutamine:fructose-6-phosphate amidotransferase	0	NULL	NULL	NULL	gw60_diabetes_50_5_1093_s_411	11334413	Diabetes 45:1644 - 1654, 1996 [Abstract]    Cooksey RC, Hebert LF, Zhu JH, Wofford P, Garvey WT, McClain DA: Mechanism of hexosamine-induced insulin resistance in transgenic mice overexpressing glutamine:fructose-6-phosphate amidotransferase: decreased glucose transporter GLUT4 translocation and reversal by treatment with thiazolidinedione.	transcription
51718	1	334851	5	NULL	NULL	0	NULL	glucose	NULL	increase in;;levels of	increases	NULL				Id2	NULL	levels of			NULL	J774.2 macrophages	0	NULL	NULL	NULL	abs-batch0620-0649_am-j-physiol-endocrinol-metab_290_4_16234270_s_7	16234270	We demonstrate that increases in glucose levels cause  a rapid increase in levels of Id2 in J774.2 macrophages, and a number  of lines of evidence indicate that this is via the hexosamine pathway  because 1) the effect of glucose requires glutamine; 2) the effect of  glucose is mimicked by low levels of glucosamine; 3) the effect of glucose  is inhibited by azaserine, an inhibitor of glutamine:fructose-6-phosphate  amidotransferase (GFAT); and 4) adenoviral mediated overexpression of  GFAT increases levels of Id2.	transcription
51719	2	334851	5	NULL	NULL	0	NULL	statement 1	NULL		via	NULL				hexosamine pathway	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_am-j-physiol-endocrinol-metab_290_4_16234270_s_7	16234270	We demonstrate that increases in glucose levels cause  a rapid increase in levels of Id2 in J774.2 macrophages, and a number  of lines of evidence indicate that this is via the hexosamine pathway  because 1) the effect of glucose requires glutamine; 2) the effect of  glucose is mimicked by low levels of glucosamine; 3) the effect of glucose  is inhibited by azaserine, an inhibitor of glutamine:fructose-6-phosphate  amidotransferase (GFAT); and 4) adenoviral mediated overexpression of  GFAT increases levels of Id2.	transcription
51720	3	334851	5	NULL	NULL	0	NULL	glucose	NULL	effect of	requires	NULL				glutamine	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_am-j-physiol-endocrinol-metab_290_4_16234270_s_7	16234270	We demonstrate that increases in glucose levels cause  a rapid increase in levels of Id2 in J774.2 macrophages, and a number  of lines of evidence indicate that this is via the hexosamine pathway  because 1) the effect of glucose requires glutamine; 2) the effect of  glucose is mimicked by low levels of glucosamine; 3) the effect of glucose  is inhibited by azaserine, an inhibitor of glutamine:fructose-6-phosphate  amidotransferase (GFAT); and 4) adenoviral mediated overexpression of  GFAT increases levels of Id2.	transcription
51721	4	334851	5	NULL	NULL	0	NULL	glucose	NULL	effect of	is mimicked by	NULL				glucosamine	NULL	low levels of			NULL		0	NULL	NULL	NULL	abs-batch0620-0649_am-j-physiol-endocrinol-metab_290_4_16234270_s_7	16234270	We demonstrate that increases in glucose levels cause  a rapid increase in levels of Id2 in J774.2 macrophages, and a number  of lines of evidence indicate that this is via the hexosamine pathway  because 1) the effect of glucose requires glutamine; 2) the effect of  glucose is mimicked by low levels of glucosamine; 3) the effect of glucose  is inhibited by azaserine, an inhibitor of glutamine:fructose-6-phosphate  amidotransferase (GFAT); and 4) adenoviral mediated overexpression of  GFAT increases levels of Id2.	transcription
51722	5	334851	5	NULL	NULL	0	NULL	glucose	NULL	effect of	is inhibited by	NULL				azaserine	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_am-j-physiol-endocrinol-metab_290_4_16234270_s_7	16234270	We demonstrate that increases in glucose levels cause  a rapid increase in levels of Id2 in J774.2 macrophages, and a number  of lines of evidence indicate that this is via the hexosamine pathway  because 1) the effect of glucose requires glutamine; 2) the effect of  glucose is mimicked by low levels of glucosamine; 3) the effect of glucose  is inhibited by azaserine, an inhibitor of glutamine:fructose-6-phosphate  amidotransferase (GFAT); and 4) adenoviral mediated overexpression of  GFAT increases levels of Id2.	transcription
51723	6	334851	5	NULL	NULL	0	NULL	azaserine	NULL		is an inhibitor of	NULL				GFAT	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_am-j-physiol-endocrinol-metab_290_4_16234270_s_7	16234270	We demonstrate that increases in glucose levels cause  a rapid increase in levels of Id2 in J774.2 macrophages, and a number  of lines of evidence indicate that this is via the hexosamine pathway  because 1) the effect of glucose requires glutamine; 2) the effect of  glucose is mimicked by low levels of glucosamine; 3) the effect of glucose  is inhibited by azaserine, an inhibitor of glutamine:fructose-6-phosphate  amidotransferase (GFAT); and 4) adenoviral mediated overexpression of  GFAT increases levels of Id2.	transcription
51724	7	334851	5	NULL	NULL	0	NULL	GFAT	NULL		is	NULL				glutamine:fructose-6-phosphate amidotransferase	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_am-j-physiol-endocrinol-metab_290_4_16234270_s_7	16234270	We demonstrate that increases in glucose levels cause  a rapid increase in levels of Id2 in J774.2 macrophages, and a number  of lines of evidence indicate that this is via the hexosamine pathway  because 1) the effect of glucose requires glutamine; 2) the effect of  glucose is mimicked by low levels of glucosamine; 3) the effect of glucose  is inhibited by azaserine, an inhibitor of glutamine:fructose-6-phosphate  amidotransferase (GFAT); and 4) adenoviral mediated overexpression of  GFAT increases levels of Id2.	transcription
51725	8	334851	5	NULL	NULL	0	NULL	adenovirus	NULL		mediate	NULL				GFAT	NULL	overexpression of			NULL		0	NULL	NULL	NULL	abs-batch0620-0649_am-j-physiol-endocrinol-metab_290_4_16234270_s_7	16234270	We demonstrate that increases in glucose levels cause  a rapid increase in levels of Id2 in J774.2 macrophages, and a number  of lines of evidence indicate that this is via the hexosamine pathway  because 1) the effect of glucose requires glutamine; 2) the effect of  glucose is mimicked by low levels of glucosamine; 3) the effect of glucose  is inhibited by azaserine, an inhibitor of glutamine:fructose-6-phosphate  amidotransferase (GFAT); and 4) adenoviral mediated overexpression of  GFAT increases levels of Id2.	transcription
51726	9	334851	5	NULL	NULL	0	NULL	statement 8	NULL		increases	NULL				Id2	NULL	levels of			NULL		0	NULL	NULL	NULL	abs-batch0620-0649_am-j-physiol-endocrinol-metab_290_4_16234270_s_7	16234270	We demonstrate that increases in glucose levels cause  a rapid increase in levels of Id2 in J774.2 macrophages, and a number  of lines of evidence indicate that this is via the hexosamine pathway  because 1) the effect of glucose requires glutamine; 2) the effect of  glucose is mimicked by low levels of glucosamine; 3) the effect of glucose  is inhibited by azaserine, an inhibitor of glutamine:fructose-6-phosphate  amidotransferase (GFAT); and 4) adenoviral mediated overexpression of  GFAT increases levels of Id2.	transcription
52541	1	334851	6	NULL	NULL	0	NULL	glucose	NULL	increased levels of 	increases	NULL				Id2	NULL	levels of 			NULL	J774.2 macrophages	0	NULL	NULL	NULL	abs-batch0620-0649_am-j-physiol-endocrinol-metab_290_4_16234270_s_7	16234270	We demonstrate that increases in glucose levels cause  a rapid increase in levels of Id2 in J774.2 macrophages, and a number  of lines of evidence indicate that this is via the hexosamine pathway  because 1) the effect of glucose requires glutamine; 2) the effect of  glucose is mimicked by low levels of glucosamine; 3) the effect of glucose  is inhibited by azaserine, an inhibitor of glutamine:fructose-6-phosphate  amidotransferase (GFAT); and 4) adenoviral mediated overexpression of  GFAT increases levels of Id2.	transcription
52542	2	334851	6	NULL	NULL	0	NULL	statement 1	NULL		occurs via	NULL				hexosamine pathway	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_am-j-physiol-endocrinol-metab_290_4_16234270_s_7	16234270	We demonstrate that increases in glucose levels cause  a rapid increase in levels of Id2 in J774.2 macrophages, and a number  of lines of evidence indicate that this is via the hexosamine pathway  because 1) the effect of glucose requires glutamine; 2) the effect of  glucose is mimicked by low levels of glucosamine; 3) the effect of glucose  is inhibited by azaserine, an inhibitor of glutamine:fructose-6-phosphate  amidotransferase (GFAT); and 4) adenoviral mediated overexpression of  GFAT increases levels of Id2.	transcription
52543	3	334851	6	NULL	NULL	0	NULL	glucose	NULL	effect of	requires	NULL				glutamine	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_am-j-physiol-endocrinol-metab_290_4_16234270_s_7	16234270	We demonstrate that increases in glucose levels cause  a rapid increase in levels of Id2 in J774.2 macrophages, and a number  of lines of evidence indicate that this is via the hexosamine pathway  because 1) the effect of glucose requires glutamine; 2) the effect of  glucose is mimicked by low levels of glucosamine; 3) the effect of glucose  is inhibited by azaserine, an inhibitor of glutamine:fructose-6-phosphate  amidotransferase (GFAT); and 4) adenoviral mediated overexpression of  GFAT increases levels of Id2.	transcription
52544	4	334851	6	NULL	NULL	0	NULL	glucose	NULL	effect of	is mimicked by	NULL				glucosamine	NULL	low levels of 			NULL		0	NULL	NULL	NULL	abs-batch0620-0649_am-j-physiol-endocrinol-metab_290_4_16234270_s_7	16234270	We demonstrate that increases in glucose levels cause  a rapid increase in levels of Id2 in J774.2 macrophages, and a number  of lines of evidence indicate that this is via the hexosamine pathway  because 1) the effect of glucose requires glutamine; 2) the effect of  glucose is mimicked by low levels of glucosamine; 3) the effect of glucose  is inhibited by azaserine, an inhibitor of glutamine:fructose-6-phosphate  amidotransferase (GFAT); and 4) adenoviral mediated overexpression of  GFAT increases levels of Id2.	transcription
52545	5	334851	6	NULL	NULL	0	NULL	azaserine	NULL		inhibits	NULL				glucose	NULL	effect of 			NULL		0	NULL	NULL	NULL	abs-batch0620-0649_am-j-physiol-endocrinol-metab_290_4_16234270_s_7	16234270	We demonstrate that increases in glucose levels cause  a rapid increase in levels of Id2 in J774.2 macrophages, and a number  of lines of evidence indicate that this is via the hexosamine pathway  because 1) the effect of glucose requires glutamine; 2) the effect of  glucose is mimicked by low levels of glucosamine; 3) the effect of glucose  is inhibited by azaserine, an inhibitor of glutamine:fructose-6-phosphate  amidotransferase (GFAT); and 4) adenoviral mediated overexpression of  GFAT increases levels of Id2.	transcription
52546	6	334851	6	NULL	NULL	0	NULL	azaserine	NULL		is a type of 	NULL				GFAT inhibitor	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_am-j-physiol-endocrinol-metab_290_4_16234270_s_7	16234270	We demonstrate that increases in glucose levels cause  a rapid increase in levels of Id2 in J774.2 macrophages, and a number  of lines of evidence indicate that this is via the hexosamine pathway  because 1) the effect of glucose requires glutamine; 2) the effect of  glucose is mimicked by low levels of glucosamine; 3) the effect of glucose  is inhibited by azaserine, an inhibitor of glutamine:fructose-6-phosphate  amidotransferase (GFAT); and 4) adenoviral mediated overexpression of  GFAT increases levels of Id2.	transcription
52547	7	334851	6	NULL	NULL	0	NULL	GFAT	NULL		is	NULL				glutamine:fructose-6-phosphate amidotransferase	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_am-j-physiol-endocrinol-metab_290_4_16234270_s_7	16234270	We demonstrate that increases in glucose levels cause  a rapid increase in levels of Id2 in J774.2 macrophages, and a number  of lines of evidence indicate that this is via the hexosamine pathway  because 1) the effect of glucose requires glutamine; 2) the effect of  glucose is mimicked by low levels of glucosamine; 3) the effect of glucose  is inhibited by azaserine, an inhibitor of glutamine:fructose-6-phosphate  amidotransferase (GFAT); and 4) adenoviral mediated overexpression of  GFAT increases levels of Id2.	transcription
51727	1	334852	5	NULL	NULL	0	NULL	glucose	NULL		up-regulates	NULL				USF-1 mRNA	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_158	14757763	To assess whether the HBP mediates glucose-induced up-regulation of both USF-1 and USF-2 mRNA, we incubated porcine mesangial cells with 2 mM glucosamine or 30 mM glucose plus 16 mM glutamine for 24 h. GFAT, the rate-limiting enzyme of the HBP, requires glutamine for conversion of fructose-6-phosphate to glucosamine-6-phosphate, whereas glucosamine enters the HBP downstream of GFAT.	transcription
51728	2	334852	5	NULL	NULL	0	NULL	glucose	NULL		up-regulates	NULL				USF-2 mRNA	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_158	14757763	To assess whether the HBP mediates glucose-induced up-regulation of both USF-1 and USF-2 mRNA, we incubated porcine mesangial cells with 2 mM glucosamine or 30 mM glucose plus 16 mM glutamine for 24 h. GFAT, the rate-limiting enzyme of the HBP, requires glutamine for conversion of fructose-6-phosphate to glucosamine-6-phosphate, whereas glucosamine enters the HBP downstream of GFAT.	transcription
51729	3	334852	5	NULL	NULL	0	NULL	GFAT	NULL		is a type of	NULL				rate-limiting enzyme of HBP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_158	14757763	To assess whether the HBP mediates glucose-induced up-regulation of both USF-1 and USF-2 mRNA, we incubated porcine mesangial cells with 2 mM glucosamine or 30 mM glucose plus 16 mM glutamine for 24 h. GFAT, the rate-limiting enzyme of the HBP, requires glutamine for conversion of fructose-6-phosphate to glucosamine-6-phosphate, whereas glucosamine enters the HBP downstream of GFAT.	transcription
51730	4	334852	5	NULL	NULL	0	NULL	fructose-6-phosphate	NULL		is converted to	NULL				glucosamine-6-phosphate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_158	14757763	To assess whether the HBP mediates glucose-induced up-regulation of both USF-1 and USF-2 mRNA, we incubated porcine mesangial cells with 2 mM glucosamine or 30 mM glucose plus 16 mM glutamine for 24 h. GFAT, the rate-limiting enzyme of the HBP, requires glutamine for conversion of fructose-6-phosphate to glucosamine-6-phosphate, whereas glucosamine enters the HBP downstream of GFAT.	transcription
51731	5	334852	5	NULL	NULL	0	NULL	GFAT	NULL		catalyzes	NULL				statement 4	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_158	14757763	To assess whether the HBP mediates glucose-induced up-regulation of both USF-1 and USF-2 mRNA, we incubated porcine mesangial cells with 2 mM glucosamine or 30 mM glucose plus 16 mM glutamine for 24 h. GFAT, the rate-limiting enzyme of the HBP, requires glutamine for conversion of fructose-6-phosphate to glucosamine-6-phosphate, whereas glucosamine enters the HBP downstream of GFAT.	transcription
51732	6	334852	5	NULL	NULL	0	NULL	glutamine	NULL		is required for	NULL				statement 5	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_158	14757763	To assess whether the HBP mediates glucose-induced up-regulation of both USF-1 and USF-2 mRNA, we incubated porcine mesangial cells with 2 mM glucosamine or 30 mM glucose plus 16 mM glutamine for 24 h. GFAT, the rate-limiting enzyme of the HBP, requires glutamine for conversion of fructose-6-phosphate to glucosamine-6-phosphate, whereas glucosamine enters the HBP downstream of GFAT.	transcription
51733	7	334852	5	NULL	NULL	0	NULL	glucosamine	NULL		enters	NULL				HBP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_158	14757763	To assess whether the HBP mediates glucose-induced up-regulation of both USF-1 and USF-2 mRNA, we incubated porcine mesangial cells with 2 mM glucosamine or 30 mM glucose plus 16 mM glutamine for 24 h. GFAT, the rate-limiting enzyme of the HBP, requires glutamine for conversion of fructose-6-phosphate to glucosamine-6-phosphate, whereas glucosamine enters the HBP downstream of GFAT.	transcription
51734	8	334852	5	NULL	NULL	0	NULL	statement 7	NULL		occurs	NULL				GFAT	NULL	downstream of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_158	14757763	To assess whether the HBP mediates glucose-induced up-regulation of both USF-1 and USF-2 mRNA, we incubated porcine mesangial cells with 2 mM glucosamine or 30 mM glucose plus 16 mM glutamine for 24 h. GFAT, the rate-limiting enzyme of the HBP, requires glutamine for conversion of fructose-6-phosphate to glucosamine-6-phosphate, whereas glucosamine enters the HBP downstream of GFAT.	transcription
52548	1	334852	6	NULL	NULL	0	NULL	glucose	NULL		mediates	NULL				USF-1 mRNA	NULL	upregulation of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_158	14757763	To assess whether the HBP mediates glucose-induced up-regulation of both USF-1 and USF-2 mRNA, we incubated porcine mesangial cells with 2 mM glucosamine or 30 mM glucose plus 16 mM glutamine for 24 h. GFAT, the rate-limiting enzyme of the HBP, requires glutamine for conversion of fructose-6-phosphate to glucosamine-6-phosphate, whereas glucosamine enters the HBP downstream of GFAT.	transcription
52549	2	334852	6	NULL	NULL	0	NULL	glucose	NULL		induces	NULL				USF-2 mRNA	NULL	upregulation of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_158	14757763	To assess whether the HBP mediates glucose-induced up-regulation of both USF-1 and USF-2 mRNA, we incubated porcine mesangial cells with 2 mM glucosamine or 30 mM glucose plus 16 mM glutamine for 24 h. GFAT, the rate-limiting enzyme of the HBP, requires glutamine for conversion of fructose-6-phosphate to glucosamine-6-phosphate, whereas glucosamine enters the HBP downstream of GFAT.	transcription
52550	3	334852	6	NULL	NULL	0	NULL	GFAT	NULL		is a type of 	NULL				HBP enzyme	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_158	14757763	To assess whether the HBP mediates glucose-induced up-regulation of both USF-1 and USF-2 mRNA, we incubated porcine mesangial cells with 2 mM glucosamine or 30 mM glucose plus 16 mM glutamine for 24 h. GFAT, the rate-limiting enzyme of the HBP, requires glutamine for conversion of fructose-6-phosphate to glucosamine-6-phosphate, whereas glucosamine enters the HBP downstream of GFAT.	transcription
52551	4	334852	6	NULL	NULL	0	NULL	fructose-6-phosphate	NULL		is converted to	NULL				glucosamine-6-phosphate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_158	14757763	To assess whether the HBP mediates glucose-induced up-regulation of both USF-1 and USF-2 mRNA, we incubated porcine mesangial cells with 2 mM glucosamine or 30 mM glucose plus 16 mM glutamine for 24 h. GFAT, the rate-limiting enzyme of the HBP, requires glutamine for conversion of fructose-6-phosphate to glucosamine-6-phosphate, whereas glucosamine enters the HBP downstream of GFAT.	transcription
52552	5	334852	6	NULL	NULL	0	NULL	glutamine	NULL		is required for	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_158	14757763	To assess whether the HBP mediates glucose-induced up-regulation of both USF-1 and USF-2 mRNA, we incubated porcine mesangial cells with 2 mM glucosamine or 30 mM glucose plus 16 mM glutamine for 24 h. GFAT, the rate-limiting enzyme of the HBP, requires glutamine for conversion of fructose-6-phosphate to glucosamine-6-phosphate, whereas glucosamine enters the HBP downstream of GFAT.	transcription
52553	6	334852	6	NULL	NULL	0	NULL	glucosamine	NULL		enters	NULL				HBP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_158	14757763	To assess whether the HBP mediates glucose-induced up-regulation of both USF-1 and USF-2 mRNA, we incubated porcine mesangial cells with 2 mM glucosamine or 30 mM glucose plus 16 mM glutamine for 24 h. GFAT, the rate-limiting enzyme of the HBP, requires glutamine for conversion of fructose-6-phosphate to glucosamine-6-phosphate, whereas glucosamine enters the HBP downstream of GFAT.	transcription
52554	7	334852	6	NULL	NULL	0	NULL	statement 6	NULL		occurs downstream of	NULL				GFAT	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15908_s_158	14757763	To assess whether the HBP mediates glucose-induced up-regulation of both USF-1 and USF-2 mRNA, we incubated porcine mesangial cells with 2 mM glucosamine or 30 mM glucose plus 16 mM glutamine for 24 h. GFAT, the rate-limiting enzyme of the HBP, requires glutamine for conversion of fructose-6-phosphate to glucosamine-6-phosphate, whereas glucosamine enters the HBP downstream of GFAT.	transcription
51735	1	334853	5	NULL	NULL	0	NULL	hyperglycemia	NULL		induce	NULL				ED	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_103_1_218_s_36	16373499	Pathophysiological mechanisms for hyperglycemia-induced ED via generation of ROS involve: ( i) protein kinase C activation, ( ii) increased generation of advanced glycation end products, ( iii) increased glucose flux through the aldose reductase pathway, ( iv) increased activity of glutamine:fructose-6-phosphate amidotransferase leading to insulin resistance, and ( v) activation of NFkappaB leading to nuclear transcription of cytokines and inflammatory mediators.	transcription
51736	2	334853	5	NULL	NULL	0	NULL	statement 1	NULL		via	NULL				ROS	NULL	generation of			NULL		0	NULL	NULL	NULL	gw70_pnas_103_1_218_s_36	16373499	Pathophysiological mechanisms for hyperglycemia-induced ED via generation of ROS involve: ( i) protein kinase C activation, ( ii) increased generation of advanced glycation end products, ( iii) increased glucose flux through the aldose reductase pathway, ( iv) increased activity of glutamine:fructose-6-phosphate amidotransferase leading to insulin resistance, and ( v) activation of NFkappaB leading to nuclear transcription of cytokines and inflammatory mediators.	transcription
51737	3	334853	5	NULL	NULL	0	NULL	statement 1	NULL		involves	NULL				protein kinase C	NULL	activation of			NULL		0	NULL	NULL	NULL	gw70_pnas_103_1_218_s_36	16373499	Pathophysiological mechanisms for hyperglycemia-induced ED via generation of ROS involve: ( i) protein kinase C activation, ( ii) increased generation of advanced glycation end products, ( iii) increased glucose flux through the aldose reductase pathway, ( iv) increased activity of glutamine:fructose-6-phosphate amidotransferase leading to insulin resistance, and ( v) activation of NFkappaB leading to nuclear transcription of cytokines and inflammatory mediators.	transcription
51738	4	334853	5	NULL	NULL	0	NULL	statement 1	NULL		involves	NULL				glycation end products	NULL	increased generation of;;advanced			NULL		0	NULL	NULL	NULL	gw70_pnas_103_1_218_s_36	16373499	Pathophysiological mechanisms for hyperglycemia-induced ED via generation of ROS involve: ( i) protein kinase C activation, ( ii) increased generation of advanced glycation end products, ( iii) increased glucose flux through the aldose reductase pathway, ( iv) increased activity of glutamine:fructose-6-phosphate amidotransferase leading to insulin resistance, and ( v) activation of NFkappaB leading to nuclear transcription of cytokines and inflammatory mediators.	transcription
51739	5	334853	5	NULL	NULL	0	NULL	statement 1	NULL		involves	NULL				glucose flux	NULL	increased			NULL		0	NULL	NULL	NULL	gw70_pnas_103_1_218_s_36	16373499	Pathophysiological mechanisms for hyperglycemia-induced ED via generation of ROS involve: ( i) protein kinase C activation, ( ii) increased generation of advanced glycation end products, ( iii) increased glucose flux through the aldose reductase pathway, ( iv) increased activity of glutamine:fructose-6-phosphate amidotransferase leading to insulin resistance, and ( v) activation of NFkappaB leading to nuclear transcription of cytokines and inflammatory mediators.	transcription
51740	6	334853	5	NULL	NULL	0	NULL	statement 5	NULL		occurs through	NULL				aldose reductase pathway	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_103_1_218_s_36	16373499	Pathophysiological mechanisms for hyperglycemia-induced ED via generation of ROS involve: ( i) protein kinase C activation, ( ii) increased generation of advanced glycation end products, ( iii) increased glucose flux through the aldose reductase pathway, ( iv) increased activity of glutamine:fructose-6-phosphate amidotransferase leading to insulin resistance, and ( v) activation of NFkappaB leading to nuclear transcription of cytokines and inflammatory mediators.	transcription
51741	7	334853	5	NULL	NULL	0	NULL	statement 1	NULL		involves	NULL				glutamine:fructose-6-phosphate amidotransferase 	NULL	increased activity of 			NULL		0	NULL	NULL	NULL	gw70_pnas_103_1_218_s_36	16373499	Pathophysiological mechanisms for hyperglycemia-induced ED via generation of ROS involve: ( i) protein kinase C activation, ( ii) increased generation of advanced glycation end products, ( iii) increased glucose flux through the aldose reductase pathway, ( iv) increased activity of glutamine:fructose-6-phosphate amidotransferase leading to insulin resistance, and ( v) activation of NFkappaB leading to nuclear transcription of cytokines and inflammatory mediators.	transcription
51742	8	334853	5	NULL	NULL	0	NULL	statement 8	NULL		leads to	NULL				insulin resistance	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_103_1_218_s_36	16373499	Pathophysiological mechanisms for hyperglycemia-induced ED via generation of ROS involve: ( i) protein kinase C activation, ( ii) increased generation of advanced glycation end products, ( iii) increased glucose flux through the aldose reductase pathway, ( iv) increased activity of glutamine:fructose-6-phosphate amidotransferase leading to insulin resistance, and ( v) activation of NFkappaB leading to nuclear transcription of cytokines and inflammatory mediators.	transcription
51743	9	334853	5	NULL	NULL	0	NULL	statement 1	NULL		involves	NULL				NF-kappaB	NULL	activation of			NULL		0	NULL	NULL	NULL	gw70_pnas_103_1_218_s_36	16373499	Pathophysiological mechanisms for hyperglycemia-induced ED via generation of ROS involve: ( i) protein kinase C activation, ( ii) increased generation of advanced glycation end products, ( iii) increased glucose flux through the aldose reductase pathway, ( iv) increased activity of glutamine:fructose-6-phosphate amidotransferase leading to insulin resistance, and ( v) activation of NFkappaB leading to nuclear transcription of cytokines and inflammatory mediators.	transcription
51744	10	334853	5	NULL	NULL	0	NULL	statement 9	NULL		leads to	NULL				cytokines	NULL	nuclear transcription of			NULL		0	NULL	NULL	NULL	gw70_pnas_103_1_218_s_36	16373499	Pathophysiological mechanisms for hyperglycemia-induced ED via generation of ROS involve: ( i) protein kinase C activation, ( ii) increased generation of advanced glycation end products, ( iii) increased glucose flux through the aldose reductase pathway, ( iv) increased activity of glutamine:fructose-6-phosphate amidotransferase leading to insulin resistance, and ( v) activation of NFkappaB leading to nuclear transcription of cytokines and inflammatory mediators.	transcription
51745	11	334853	5	NULL	NULL	0	NULL	statement 9	NULL		leads to	NULL				inflammatory mediators	NULL	nuclear transcription of			NULL		0	NULL	NULL	NULL	gw70_pnas_103_1_218_s_36	16373499	Pathophysiological mechanisms for hyperglycemia-induced ED via generation of ROS involve: ( i) protein kinase C activation, ( ii) increased generation of advanced glycation end products, ( iii) increased glucose flux through the aldose reductase pathway, ( iv) increased activity of glutamine:fructose-6-phosphate amidotransferase leading to insulin resistance, and ( v) activation of NFkappaB leading to nuclear transcription of cytokines and inflammatory mediators.	transcription
52962	1	334853	6	NULL	NULL	0	NULL	hyperglycemia	NULL		induce	NULL				ED	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_103_1_218_s_36	16373499	Pathophysiological mechanisms for hyperglycemia-induced ED via generation of ROS involve: ( i) protein kinase C activation, ( ii) increased generation of advanced glycation end products, ( iii) increased glucose flux through the aldose reductase pathway, ( iv) increased activity of glutamine:fructose-6-phosphate amidotransferase leading to insulin resistance, and ( v) activation of NFkappaB leading to nuclear transcription of cytokines and inflammatory mediators.	transcription
52963	2	334853	6	NULL	NULL	0	NULL	statement 1	NULL		occurs via	NULL				ROS	NULL	generation of 			NULL		0	NULL	NULL	NULL	gw70_pnas_103_1_218_s_36	16373499	Pathophysiological mechanisms for hyperglycemia-induced ED via generation of ROS involve: ( i) protein kinase C activation, ( ii) increased generation of advanced glycation end products, ( iii) increased glucose flux through the aldose reductase pathway, ( iv) increased activity of glutamine:fructose-6-phosphate amidotransferase leading to insulin resistance, and ( v) activation of NFkappaB leading to nuclear transcription of cytokines and inflammatory mediators.	transcription
52964	3	334853	6	NULL	NULL	0	NULL	statement 1	NULL		involve	NULL				protein kinase C	NULL	activation of			NULL		0	NULL	NULL	NULL	gw70_pnas_103_1_218_s_36	16373499	Pathophysiological mechanisms for hyperglycemia-induced ED via generation of ROS involve: ( i) protein kinase C activation, ( ii) increased generation of advanced glycation end products, ( iii) increased glucose flux through the aldose reductase pathway, ( iv) increased activity of glutamine:fructose-6-phosphate amidotransferase leading to insulin resistance, and ( v) activation of NFkappaB leading to nuclear transcription of cytokines and inflammatory mediators.	transcription
52965	4	334853	6	NULL	NULL	0	NULL	statement 1	NULL		involve	NULL				glycation end products	NULL	increased generation of;; advanced			NULL		0	NULL	NULL	NULL	gw70_pnas_103_1_218_s_36	16373499	Pathophysiological mechanisms for hyperglycemia-induced ED via generation of ROS involve: ( i) protein kinase C activation, ( ii) increased generation of advanced glycation end products, ( iii) increased glucose flux through the aldose reductase pathway, ( iv) increased activity of glutamine:fructose-6-phosphate amidotransferase leading to insulin resistance, and ( v) activation of NFkappaB leading to nuclear transcription of cytokines and inflammatory mediators.	transcription
52966	5	334853	6	NULL	NULL	0	NULL	statement 1	NULL		involves	NULL				glucose flux	NULL	increased			NULL		0	NULL	NULL	NULL	gw70_pnas_103_1_218_s_36	16373499	Pathophysiological mechanisms for hyperglycemia-induced ED via generation of ROS involve: ( i) protein kinase C activation, ( ii) increased generation of advanced glycation end products, ( iii) increased glucose flux through the aldose reductase pathway, ( iv) increased activity of glutamine:fructose-6-phosphate amidotransferase leading to insulin resistance, and ( v) activation of NFkappaB leading to nuclear transcription of cytokines and inflammatory mediators.	transcription
52967	6	334853	6	NULL	NULL	0	NULL	statement 5	NULL		occurs through	NULL				aldose reductase pathway	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_103_1_218_s_36	16373499	Pathophysiological mechanisms for hyperglycemia-induced ED via generation of ROS involve: ( i) protein kinase C activation, ( ii) increased generation of advanced glycation end products, ( iii) increased glucose flux through the aldose reductase pathway, ( iv) increased activity of glutamine:fructose-6-phosphate amidotransferase leading to insulin resistance, and ( v) activation of NFkappaB leading to nuclear transcription of cytokines and inflammatory mediators.	transcription
52968	7	334853	6	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				glutamine:fructose-6-phosphate amidotransferase	NULL	increased activity of 			NULL		0	NULL	NULL	NULL	gw70_pnas_103_1_218_s_36	16373499	Pathophysiological mechanisms for hyperglycemia-induced ED via generation of ROS involve: ( i) protein kinase C activation, ( ii) increased generation of advanced glycation end products, ( iii) increased glucose flux through the aldose reductase pathway, ( iv) increased activity of glutamine:fructose-6-phosphate amidotransferase leading to insulin resistance, and ( v) activation of NFkappaB leading to nuclear transcription of cytokines and inflammatory mediators.	transcription
52969	8	334853	6	NULL	NULL	0	NULL	statement 7	NULL		leads to	NULL				insulin resistance	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_103_1_218_s_36	16373499	Pathophysiological mechanisms for hyperglycemia-induced ED via generation of ROS involve: ( i) protein kinase C activation, ( ii) increased generation of advanced glycation end products, ( iii) increased glucose flux through the aldose reductase pathway, ( iv) increased activity of glutamine:fructose-6-phosphate amidotransferase leading to insulin resistance, and ( v) activation of NFkappaB leading to nuclear transcription of cytokines and inflammatory mediators.	transcription
52970	9	334853	6	NULL	NULL	0	NULL	statement 1	NULL		involves	NULL				NFkappaB	NULL	activation of			NULL		0	NULL	NULL	NULL	gw70_pnas_103_1_218_s_36	16373499	Pathophysiological mechanisms for hyperglycemia-induced ED via generation of ROS involve: ( i) protein kinase C activation, ( ii) increased generation of advanced glycation end products, ( iii) increased glucose flux through the aldose reductase pathway, ( iv) increased activity of glutamine:fructose-6-phosphate amidotransferase leading to insulin resistance, and ( v) activation of NFkappaB leading to nuclear transcription of cytokines and inflammatory mediators.	transcription
52971	10	334853	6	NULL	NULL	0	NULL	statement 9	NULL		leads to	NULL				cytokines	NULL	nuclear transcription of 			NULL		0	NULL	NULL	NULL	gw70_pnas_103_1_218_s_36	16373499	Pathophysiological mechanisms for hyperglycemia-induced ED via generation of ROS involve: ( i) protein kinase C activation, ( ii) increased generation of advanced glycation end products, ( iii) increased glucose flux through the aldose reductase pathway, ( iv) increased activity of glutamine:fructose-6-phosphate amidotransferase leading to insulin resistance, and ( v) activation of NFkappaB leading to nuclear transcription of cytokines and inflammatory mediators.	transcription
52972	11	334853	6	NULL	NULL	0	NULL	statement 9	NULL		leads to	NULL				inflammatory cytokines	NULL	nuclear transcription of			NULL		0	NULL	NULL	NULL	gw70_pnas_103_1_218_s_36	16373499	Pathophysiological mechanisms for hyperglycemia-induced ED via generation of ROS involve: ( i) protein kinase C activation, ( ii) increased generation of advanced glycation end products, ( iii) increased glucose flux through the aldose reductase pathway, ( iv) increased activity of glutamine:fructose-6-phosphate amidotransferase leading to insulin resistance, and ( v) activation of NFkappaB leading to nuclear transcription of cytokines and inflammatory mediators.	transcription
51746	1	334854	5	NULL	NULL	0	NULL	OXA-10 enzyme	NULL		bind	NULL				metal	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1546_1_132_s_216	11257516	In both OXA-2 and -3, the histidine and one of the two glutamates involved in metal binding in OXA-10 enzyme are replaced by arginine and aspartate, respectively.	transcription
51747	2	334854	5	NULL	NULL	0	NULL	histidine	NULL		is involved in	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1546_1_132_s_216	11257516	In both OXA-2 and -3, the histidine and one of the two glutamates involved in metal binding in OXA-10 enzyme are replaced by arginine and aspartate, respectively.	transcription
51748	3	334854	5	NULL	NULL	0	NULL	glutamate	NULL		is involved in	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1546_1_132_s_216	11257516	In both OXA-2 and -3, the histidine and one of the two glutamates involved in metal binding in OXA-10 enzyme are replaced by arginine and aspartate, respectively.	transcription
52555	1	334855	6	NULL	NULL	0	NULL		NULL		produces	NULL		V67K		inhibitory effect	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_26_24108_s_95	11313347	On the other hand, an additional positive charge (V67K) produces a clear inhibitory effect (Fig.  3 c) consistent with the effects of the mutations replacing glutamates/aspartates with lysines/histidines ( 9).	transcription
51749	1	334856	5	NULL	NULL	0	NULL	L-glutamate	NULL	uptake of	is inhibited by	NULL				D-leucine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_15_4071_s_160	12107123	Uptake of L-glutamate was inhibited by D-leucine, D-alanine, D-histidine, and D-alpha-aminobutyrate, but not by D-glutamate.	transcription
51750	2	334856	5	NULL	NULL	0	NULL	L-glutamate	NULL	uptake of	is inhibited by	NULL				D-alanine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_15_4071_s_160	12107123	Uptake of L-glutamate was inhibited by D-leucine, D-alanine, D-histidine, and D-alpha-aminobutyrate, but not by D-glutamate.	transcription
51751	3	334856	5	NULL	NULL	0	NULL	L-glutamate	NULL	uptake of	is inhibited by	NULL				D-histidine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_15_4071_s_160	12107123	Uptake of L-glutamate was inhibited by D-leucine, D-alanine, D-histidine, and D-alpha-aminobutyrate, but not by D-glutamate.	transcription
51752	4	334856	5	NULL	NULL	0	NULL	L-glutamate	NULL	uptake of	is inhibited by	NULL				D-alpha-aminobutyrate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_15_4071_s_160	12107123	Uptake of L-glutamate was inhibited by D-leucine, D-alanine, D-histidine, and D-alpha-aminobutyrate, but not by D-glutamate.	transcription
51753	5	334856	5	NULL	NULL	0	NULL	L-glutamate	NULL	uptake of	is not inhibited by	NULL				D-glutamate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_15_4071_s_160	12107123	Uptake of L-glutamate was inhibited by D-leucine, D-alanine, D-histidine, and D-alpha-aminobutyrate, but not by D-glutamate.	transcription
52556	1	334856	6	NULL	NULL	0	NULL	D-leucine	NULL		inhibits	NULL				L-glutamate	NULL	uptake of 			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_15_4071_s_160	12107123	Uptake of L-glutamate was inhibited by D-leucine, D-alanine, D-histidine, and D-alpha-aminobutyrate, but not by D-glutamate.	transcription
52557	2	334856	6	NULL	NULL	0	NULL	D-alanine	NULL		inhibits	NULL				L-glutamate	NULL	uptake of 			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_15_4071_s_160	12107123	Uptake of L-glutamate was inhibited by D-leucine, D-alanine, D-histidine, and D-alpha-aminobutyrate, but not by D-glutamate.	transcription
52558	3	334856	6	NULL	NULL	0	NULL	D-histidine	NULL		inhibits	NULL				L-glutamate	NULL	uptake of 			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_15_4071_s_160	12107123	Uptake of L-glutamate was inhibited by D-leucine, D-alanine, D-histidine, and D-alpha-aminobutyrate, but not by D-glutamate.	transcription
52559	4	334856	6	NULL	NULL	0	NULL	 D-alpha-aminobutyrate	NULL		inhibits	NULL				L-glutamate	NULL	uptake of 			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_15_4071_s_160	12107123	Uptake of L-glutamate was inhibited by D-leucine, D-alanine, D-histidine, and D-alpha-aminobutyrate, but not by D-glutamate.	transcription
52560	5	334856	6	NULL	NULL	0	NULL	D-glutamate	NULL		does not inhibit	NULL				L-glutamate	NULL	uptake of 			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_15_4071_s_160	12107123	Uptake of L-glutamate was inhibited by D-leucine, D-alanine, D-histidine, and D-alpha-aminobutyrate, but not by D-glutamate.	transcription
51754	1	334857	5	NULL	NULL	0	NULL	RPE65	NULL	mutant	abolishes	NULL		histidine residues;;glutamate residues		RPE65	NULL	isomerohydrolase activity of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_5_2835_s_232	16319067	However, recent studies demonstrated that mutations at the conserved histidine and glutamate residues in RPE65 abolish its isomerohydrolase activity, suggesting that these conserved histidine and aspartate/glutamate residues may be located in the iron-binding site in RPE65 ( ,  ).	transcription
51755	2	334857	5	NULL	NULL	0	NULL	RPE65	NULL		is located in	NULL	may be	histidine residues;;glutamate residues		RPE65	NULL		iron-binding site		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_5_2835_s_232	16319067	However, recent studies demonstrated that mutations at the conserved histidine and glutamate residues in RPE65 abolish its isomerohydrolase activity, suggesting that these conserved histidine and aspartate/glutamate residues may be located in the iron-binding site in RPE65 ( ,  ).	transcription
52561	1	334857	6	NULL	NULL	0	NULL	RPE65	NULL		exhibits	NULL				isomerohydrolase activity	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_5_2835_s_232	16319067	However, recent studies demonstrated that mutations at the conserved histidine and glutamate residues in RPE65 abolish its isomerohydrolase activity, suggesting that these conserved histidine and aspartate/glutamate residues may be located in the iron-binding site in RPE65 ( ,  ).	transcription
52562	2	334857	6	NULL	NULL	0	NULL	RPE65	NULL	mutation of	abolishes	NULL		hisitdine residues		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_5_2835_s_232	16319067	However, recent studies demonstrated that mutations at the conserved histidine and glutamate residues in RPE65 abolish its isomerohydrolase activity, suggesting that these conserved histidine and aspartate/glutamate residues may be located in the iron-binding site in RPE65 ( ,  ).	transcription
52563	3	334857	6	NULL	NULL	0	NULL	RPE65	NULL	mutation of	abolishes	NULL		glutamate residues		statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_5_2835_s_232	16319067	However, recent studies demonstrated that mutations at the conserved histidine and glutamate residues in RPE65 abolish its isomerohydrolase activity, suggesting that these conserved histidine and aspartate/glutamate residues may be located in the iron-binding site in RPE65 ( ,  ).	transcription
51759	1	334858	5	NULL	NULL	0	NULL	histidine	NULL		block	NULL				3H-glutamine	NULL	transport of 			NULL	transfected cells	0	NULL	NULL	NULL	gw60_cell_99_7_769_s_158	10619430	Similar concentrations of  histidine block the transport of 3H-glutamine by transfected and untransfected cells whereas  glutamate has little effect on either.	transcription
51760	2	334858	5	NULL	NULL	0	NULL	histidine	NULL		block	NULL				3H-glutamine	NULL	transport of			NULL	untransfected cells	0	NULL	NULL	NULL	gw60_cell_99_7_769_s_158	10619430	Similar concentrations of  histidine block the transport of 3H-glutamine by transfected and untransfected cells whereas  glutamate has little effect on either.	transcription
52564	1	334858	6	NULL	NULL	0	NULL	hisitidine	NULL		blocks	NULL				3H-glutamine	NULL	transport of 			NULL		0	NULL	NULL	NULL	gw60_cell_99_7_769_s_158	10619430	Similar concentrations of  histidine block the transport of 3H-glutamine by transfected and untransfected cells whereas  glutamate has little effect on either.	transcription
51761	1	334859	5	NULL	NULL	0	NULL	L-histidine	NULL		does not inhibit	NULL				L-[14]leucine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_15_4071_s_253	12107123	Also, uptake of L-[14]leucine was not inhibited by L-histidine, L-glutamate, L-glutamine, or L-proline ( 23).	transcription
51762	2	334859	5	NULL	NULL	0	NULL	L-glutamate	NULL		does not inhibit	NULL				L-[14]leucine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_15_4071_s_253	12107123	Also, uptake of L-[14]leucine was not inhibited by L-histidine, L-glutamate, L-glutamine, or L-proline ( 23).	transcription
51763	3	334859	5	NULL	NULL	0	NULL	L-glutamine	NULL		does not inhibit	NULL				L-[14]leucine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_15_4071_s_253	12107123	Also, uptake of L-[14]leucine was not inhibited by L-histidine, L-glutamate, L-glutamine, or L-proline ( 23).	transcription
51764	4	334859	5	NULL	NULL	0	NULL	L-proline	NULL		does not inhibit	NULL				L-[14]leucine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_15_4071_s_253	12107123	Also, uptake of L-[14]leucine was not inhibited by L-histidine, L-glutamate, L-glutamine, or L-proline ( 23).	transcription
52565	1	334859	6	NULL	NULL	0	NULL	L-histidine	NULL		does not inhibit	NULL				L-[14]leucine	NULL	uptake of 			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_15_4071_s_253	12107123	Also, uptake of L-[14]leucine was not inhibited by L-histidine, L-glutamate, L-glutamine, or L-proline ( 23).	transcription
52566	2	334859	6	NULL	NULL	0	NULL	L-glutamate	NULL		does not inhibit	NULL				L-[14]leucine	NULL	uptake of 			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_15_4071_s_253	12107123	Also, uptake of L-[14]leucine was not inhibited by L-histidine, L-glutamate, L-glutamine, or L-proline ( 23).	transcription
52567	3	334859	6	NULL	NULL	0	NULL	L-glutamine	NULL		does not inhibit	NULL				L-[14]leucine	NULL	uptake of 			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_15_4071_s_253	12107123	Also, uptake of L-[14]leucine was not inhibited by L-histidine, L-glutamate, L-glutamine, or L-proline ( 23).	transcription
52568	4	334859	6	NULL	NULL	0	NULL	 L-proline	NULL		does not inhibit	NULL				L-[14]leucine	NULL	uptake of 			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_15_4071_s_253	12107123	Also, uptake of L-[14]leucine was not inhibited by L-histidine, L-glutamate, L-glutamine, or L-proline ( 23).	transcription
52569	1	334860	6	NULL	NULL	0	NULL	EAAT1	NULL		includes	NULL		Zn2+ binding site			NULL		histidine residues		NULL		0	NULL	NULL	NULL	gw60_molpharmacol_54_1_189_s_158	9658205	Thus, it may be concluded that the Zn2+ binding site on EAAT1 includes two histidine residues and the differential inhibition of glutamate transporter subtypes may be explained by the presence or absence of a histidine residue corresponding to position 156 of EAAT1.	transcription
51788	1	334861	5	NULL	NULL	0	NULL	glycine	NULL	conserved	allows	NULL				beta-turn	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_31_28280_s_250	12034745	The glutamate is required for catalysis, and the conserved glycine allows the formation of a beta-turn that brings the zinc ligands together; in addition, water is used as a nucleophile, which is bound by a single zinc ion ligated to the three histidines ( 26).	transcription
51789	2	334861	5	NULL	NULL	0	NULL	beta-turn	NULL		brings together	NULL				zinc ligands	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_31_28280_s_250	12034745	The glutamate is required for catalysis, and the conserved glycine allows the formation of a beta-turn that brings the zinc ligands together; in addition, water is used as a nucleophile, which is bound by a single zinc ion ligated to the three histidines ( 26).	transcription
51790	3	334861	5	NULL	NULL	0	NULL	water	NULL		acts as	NULL				nucleophile	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_31_28280_s_250	12034745	The glutamate is required for catalysis, and the conserved glycine allows the formation of a beta-turn that brings the zinc ligands together; in addition, water is used as a nucleophile, which is bound by a single zinc ion ligated to the three histidines ( 26).	transcription
51791	4	334861	5	NULL	NULL	0	NULL	zinc ion	NULL	single	is ligated to	NULL				histidines	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_31_28280_s_250	12034745	The glutamate is required for catalysis, and the conserved glycine allows the formation of a beta-turn that brings the zinc ligands together; in addition, water is used as a nucleophile, which is bound by a single zinc ion ligated to the three histidines ( 26).	transcription
51792	5	334861	5	NULL	NULL	0	NULL	water	NULL		is bound by	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_31_28280_s_250	12034745	The glutamate is required for catalysis, and the conserved glycine allows the formation of a beta-turn that brings the zinc ligands together; in addition, water is used as a nucleophile, which is bound by a single zinc ion ligated to the three histidines ( 26).	transcription
52570	1	334861	6	NULL	NULL	0	NULL	zinc ion	NULL	single	is ligated to	NULL				histidine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_31_28280_s_250	12034745	The glutamate is required for catalysis, and the conserved glycine allows the formation of a beta-turn that brings the zinc ligands together; in addition, water is used as a nucleophile, which is bound by a single zinc ion ligated to the three histidines ( 26).	transcription
52571	2	334861	6	NULL	NULL	0	NULL	water	NULL		bind	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_31_28280_s_250	12034745	The glutamate is required for catalysis, and the conserved glycine allows the formation of a beta-turn that brings the zinc ligands together; in addition, water is used as a nucleophile, which is bound by a single zinc ion ligated to the three histidines ( 26).	transcription
52572	3	334861	6	NULL	NULL	0	NULL	glycine	NULL	conserved	allows	NULL					NULL	formation of	beta-turn		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_31_28280_s_250	12034745	The glutamate is required for catalysis, and the conserved glycine allows the formation of a beta-turn that brings the zinc ligands together; in addition, water is used as a nucleophile, which is bound by a single zinc ion ligated to the three histidines ( 26).	transcription
52573	4	334861	6	NULL	NULL	0	NULL	statement 3	NULL		brings together	NULL				zinc ligands 	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_31_28280_s_250	12034745	The glutamate is required for catalysis, and the conserved glycine allows the formation of a beta-turn that brings the zinc ligands together; in addition, water is used as a nucleophile, which is bound by a single zinc ion ligated to the three histidines ( 26).	transcription
51793	1	334862	5	NULL	NULL	0	NULL	glutamate	NULL		plays a role in	NULL				idiophase conditions	NULL	generation of			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_67_6_2596_s_175	11375168	Study of NAD- and NADP-glutamate dehydrogenase showed that glutamate and histidine play a key role in generation of idiophase conditions by the formation of alpha-ketoglutarate, which stimulates aflatoxin formation by inhibition of the tricarboxylic acid cycle ( 3).	transcription
51794	2	334862	5	NULL	NULL	0	NULL	histidine	NULL		plays a role in	NULL				idiophase conditions	NULL	generation of			NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_67_6_2596_s_175	11375168	Study of NAD- and NADP-glutamate dehydrogenase showed that glutamate and histidine play a key role in generation of idiophase conditions by the formation of alpha-ketoglutarate, which stimulates aflatoxin formation by inhibition of the tricarboxylic acid cycle ( 3).	transcription
51795	3	334862	5	NULL	NULL	0	NULL	statement 1	NULL		occurs by	NULL				alpha-ketoglutarate	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_67_6_2596_s_175	11375168	Study of NAD- and NADP-glutamate dehydrogenase showed that glutamate and histidine play a key role in generation of idiophase conditions by the formation of alpha-ketoglutarate, which stimulates aflatoxin formation by inhibition of the tricarboxylic acid cycle ( 3).	transcription
51796	4	334862	5	NULL	NULL	0	NULL	statement 2	NULL		occurs by	NULL				alpha-ketoglutarate	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_67_6_2596_s_175	11375168	Study of NAD- and NADP-glutamate dehydrogenase showed that glutamate and histidine play a key role in generation of idiophase conditions by the formation of alpha-ketoglutarate, which stimulates aflatoxin formation by inhibition of the tricarboxylic acid cycle ( 3).	transcription
51797	5	334862	5	NULL	NULL	0	NULL	alpha-ketoglutarate	NULL		inhibits	NULL				tricarboxylic acid cycle	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_67_6_2596_s_175	11375168	Study of NAD- and NADP-glutamate dehydrogenase showed that glutamate and histidine play a key role in generation of idiophase conditions by the formation of alpha-ketoglutarate, which stimulates aflatoxin formation by inhibition of the tricarboxylic acid cycle ( 3).	transcription
51798	6	334862	5	NULL	NULL	0	NULL	statement 5	NULL		stimulates	NULL				aflatoxin	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_67_6_2596_s_175	11375168	Study of NAD- and NADP-glutamate dehydrogenase showed that glutamate and histidine play a key role in generation of idiophase conditions by the formation of alpha-ketoglutarate, which stimulates aflatoxin formation by inhibition of the tricarboxylic acid cycle ( 3).	transcription
52574	1	334862	6	NULL	NULL	0	NULL	glutamate	NULL		plays a role in	NULL				alpha-ketoglutarate	NULL	formation of 			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_67_6_2596_s_175	11375168	Study of NAD- and NADP-glutamate dehydrogenase showed that glutamate and histidine play a key role in generation of idiophase conditions by the formation of alpha-ketoglutarate, which stimulates aflatoxin formation by inhibition of the tricarboxylic acid cycle ( 3).	transcription
52575	2	334862	6	NULL	NULL	0	NULL	histidine	NULL		plays a role in	NULL				alpha-ketoglutarate	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_67_6_2596_s_175	11375168	Study of NAD- and NADP-glutamate dehydrogenase showed that glutamate and histidine play a key role in generation of idiophase conditions by the formation of alpha-ketoglutarate, which stimulates aflatoxin formation by inhibition of the tricarboxylic acid cycle ( 3).	transcription
52576	3	334862	6	NULL	NULL	0	NULL	statement 1	NULL		stimulates	NULL				aflatoxin	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_67_6_2596_s_175	11375168	Study of NAD- and NADP-glutamate dehydrogenase showed that glutamate and histidine play a key role in generation of idiophase conditions by the formation of alpha-ketoglutarate, which stimulates aflatoxin formation by inhibition of the tricarboxylic acid cycle ( 3).	transcription
52577	4	334862	6	NULL	NULL	0	NULL	statement 3	NULL		occurs via 	NULL				tricarboxylic acid cycle	NULL	inhibition of 			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_67_6_2596_s_175	11375168	Study of NAD- and NADP-glutamate dehydrogenase showed that glutamate and histidine play a key role in generation of idiophase conditions by the formation of alpha-ketoglutarate, which stimulates aflatoxin formation by inhibition of the tricarboxylic acid cycle ( 3).	transcription
52578	5	334862	6	NULL	NULL	0	NULL	statement 2	NULL		stimulates	NULL				aflatoxin	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_67_6_2596_s_175	11375168	Study of NAD- and NADP-glutamate dehydrogenase showed that glutamate and histidine play a key role in generation of idiophase conditions by the formation of alpha-ketoglutarate, which stimulates aflatoxin formation by inhibition of the tricarboxylic acid cycle ( 3).	transcription
52579	6	334862	6	NULL	NULL	0	NULL	statement 4	NULL		occurs via	NULL				tricarboxylic acid cycle	NULL	inhibition of 			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_67_6_2596_s_175	11375168	Study of NAD- and NADP-glutamate dehydrogenase showed that glutamate and histidine play a key role in generation of idiophase conditions by the formation of alpha-ketoglutarate, which stimulates aflatoxin formation by inhibition of the tricarboxylic acid cycle ( 3).	transcription
51799	1	334863	5	NULL	NULL	0	NULL	glutamate	NULL		repress	NULL					NULL	expression of		GOGAT	NULL	Salmonella typhimurium	NULL	NULL	NULL	NULL	gw60_applenvironmicrob_65_3_1099_s_319	0010049869	The observation that glutamate or glutamate-generating nitrogen substrates (arginine, proline, or histidine) repress GOGAT expression in  Salmonella typhimurium and  Klebsiella aerogenes during N-limited growth ( 6,  7) is in agreement with this hypothesis.	transcription
51800	2	334863	5	NULL	NULL	0	NULL	glutamate	NULL		repress	NULL					NULL	expression of		GOGAT	NULL	Klebsiella aerogenes	0	NULL	NULL	NULL	gw60_applenvironmicrob_65_3_1099_s_319	0010049869	The observation that glutamate or glutamate-generating nitrogen substrates (arginine, proline, or histidine) repress GOGAT expression in  Salmonella typhimurium and  Klebsiella aerogenes during N-limited growth ( 6,  7) is in agreement with this hypothesis.	transcription
51801	3	334863	5	NULL	NULL	0	NULL	statement 1	NULL		occurs during	NULL				N-limited growth	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_3_1099_s_319	0010049869	The observation that glutamate or glutamate-generating nitrogen substrates (arginine, proline, or histidine) repress GOGAT expression in  Salmonella typhimurium and  Klebsiella aerogenes during N-limited growth ( 6,  7) is in agreement with this hypothesis.	transcription
51802	4	334863	5	NULL	NULL	0	NULL	statement 2	NULL		occurs during	NULL				N-limited growth	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_3_1099_s_319	0010049869	The observation that glutamate or glutamate-generating nitrogen substrates (arginine, proline, or histidine) repress GOGAT expression in  Salmonella typhimurium and  Klebsiella aerogenes during N-limited growth ( 6,  7) is in agreement with this hypothesis.	transcription
51803	5	334863	5	NULL	NULL	0	NULL	arginine	NULL		is a type of	NULL				glutamate-generating nitrogen substrates	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_3_1099_s_319	0010049869	The observation that glutamate or glutamate-generating nitrogen substrates (arginine, proline, or histidine) repress GOGAT expression in  Salmonella typhimurium and  Klebsiella aerogenes during N-limited growth ( 6,  7) is in agreement with this hypothesis.	transcription
51804	6	334863	5	NULL	NULL	0	NULL	proline	NULL		is a type of	NULL				glutamate-generating nitrogen substrates	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_3_1099_s_319	0010049869	The observation that glutamate or glutamate-generating nitrogen substrates (arginine, proline, or histidine) repress GOGAT expression in  Salmonella typhimurium and  Klebsiella aerogenes during N-limited growth ( 6,  7) is in agreement with this hypothesis.	transcription
51805	7	334863	5	NULL	NULL	0	NULL	histidine	NULL		is a type of	NULL				glutamate-generating nitrogen substrates	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_3_1099_s_319	0010049869	The observation that glutamate or glutamate-generating nitrogen substrates (arginine, proline, or histidine) repress GOGAT expression in  Salmonella typhimurium and  Klebsiella aerogenes during N-limited growth ( 6,  7) is in agreement with this hypothesis.	transcription
51806	8	334863	5	NULL	NULL	0	NULL	arginine	NULL		repress	NULL					NULL	expression of		GOGAT	NULL	Salmonella typhimurium	NULL	NULL	NULL	NULL	gw60_applenvironmicrob_65_3_1099_s_319	0010049869	The observation that glutamate or glutamate-generating nitrogen substrates (arginine, proline, or histidine) repress GOGAT expression in  Salmonella typhimurium and  Klebsiella aerogenes during N-limited growth ( 6,  7) is in agreement with this hypothesis.	transcription
51807	9	334863	5	NULL	NULL	0	NULL	arginine	NULL		repress	NULL					NULL	expression of		GOGAT	NULL	Klebsiella aerogenes	0	NULL	NULL	NULL	gw60_applenvironmicrob_65_3_1099_s_319	0010049869	The observation that glutamate or glutamate-generating nitrogen substrates (arginine, proline, or histidine) repress GOGAT expression in  Salmonella typhimurium and  Klebsiella aerogenes during N-limited growth ( 6,  7) is in agreement with this hypothesis.	transcription
51808	10	334863	5	NULL	NULL	0	NULL	statement 8	NULL		occurs during	NULL				N-limited growth	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_3_1099_s_319	0010049869	The observation that glutamate or glutamate-generating nitrogen substrates (arginine, proline, or histidine) repress GOGAT expression in  Salmonella typhimurium and  Klebsiella aerogenes during N-limited growth ( 6,  7) is in agreement with this hypothesis.	transcription
51809	11	334863	5	NULL	NULL	0	NULL	statement 9	NULL		occurs during	NULL				N-limited growth	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_3_1099_s_319	0010049869	The observation that glutamate or glutamate-generating nitrogen substrates (arginine, proline, or histidine) repress GOGAT expression in  Salmonella typhimurium and  Klebsiella aerogenes during N-limited growth ( 6,  7) is in agreement with this hypothesis.	transcription
51810	12	334863	5	NULL	NULL	0	NULL	proline	NULL		repress	NULL					NULL	expression of		GOGAT	NULL	Salmonella typhimurium	0	NULL	NULL	NULL	gw60_applenvironmicrob_65_3_1099_s_319	0010049869	The observation that glutamate or glutamate-generating nitrogen substrates (arginine, proline, or histidine) repress GOGAT expression in  Salmonella typhimurium and  Klebsiella aerogenes during N-limited growth ( 6,  7) is in agreement with this hypothesis.	transcription
51811	13	334863	5	NULL	NULL	0	NULL	proline	NULL		repress	NULL					NULL	expression of		GOGAT	NULL	Klebsiella aerogenes	0	NULL	NULL	NULL	gw60_applenvironmicrob_65_3_1099_s_319	0010049869	The observation that glutamate or glutamate-generating nitrogen substrates (arginine, proline, or histidine) repress GOGAT expression in  Salmonella typhimurium and  Klebsiella aerogenes during N-limited growth ( 6,  7) is in agreement with this hypothesis.	transcription
51812	14	334863	5	NULL	NULL	0	NULL	statement 12	NULL		occurs during	NULL				N-limited growth	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_3_1099_s_319	0010049869	The observation that glutamate or glutamate-generating nitrogen substrates (arginine, proline, or histidine) repress GOGAT expression in  Salmonella typhimurium and  Klebsiella aerogenes during N-limited growth ( 6,  7) is in agreement with this hypothesis.	transcription
51813	15	334863	5	NULL	NULL	0	NULL	statement 13	NULL		occurs during	NULL				N-limited growth	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_3_1099_s_319	0010049869	The observation that glutamate or glutamate-generating nitrogen substrates (arginine, proline, or histidine) repress GOGAT expression in  Salmonella typhimurium and  Klebsiella aerogenes during N-limited growth ( 6,  7) is in agreement with this hypothesis.	transcription
51814	16	334863	5	NULL	NULL	0	NULL	histidine	NULL		repress	NULL					NULL	expression of		GOGAT	NULL	Salmonella typhimurium	0	NULL	NULL	NULL	gw60_applenvironmicrob_65_3_1099_s_319	0010049869	The observation that glutamate or glutamate-generating nitrogen substrates (arginine, proline, or histidine) repress GOGAT expression in  Salmonella typhimurium and  Klebsiella aerogenes during N-limited growth ( 6,  7) is in agreement with this hypothesis.	transcription
51815	17	334863	5	NULL	NULL	0	NULL	histidine	NULL		repress	NULL					NULL	expression of		GOGAT	NULL	Klebsiella aerogenes	0	NULL	NULL	NULL	gw60_applenvironmicrob_65_3_1099_s_319	0010049869	The observation that glutamate or glutamate-generating nitrogen substrates (arginine, proline, or histidine) repress GOGAT expression in  Salmonella typhimurium and  Klebsiella aerogenes during N-limited growth ( 6,  7) is in agreement with this hypothesis.	transcription
51816	18	334863	5	NULL	NULL	0	NULL	statement 16	NULL		occurs during	NULL				N-limited growth	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_3_1099_s_319	0010049869	The observation that glutamate or glutamate-generating nitrogen substrates (arginine, proline, or histidine) repress GOGAT expression in  Salmonella typhimurium and  Klebsiella aerogenes during N-limited growth ( 6,  7) is in agreement with this hypothesis.	transcription
51817	19	334863	5	NULL	NULL	0	NULL	statement 17	NULL		occurs during	NULL				N-limited growth	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_3_1099_s_319	0010049869	The observation that glutamate or glutamate-generating nitrogen substrates (arginine, proline, or histidine) repress GOGAT expression in  Salmonella typhimurium and  Klebsiella aerogenes during N-limited growth ( 6,  7) is in agreement with this hypothesis.	transcription
52580	1	334863	6	NULL	NULL	0	NULL	glutamate	NULL		repress	NULL				GOGAT	NULL	expression of 			NULL	Salmonella typhimurium	0	NULL	NULL	NULL	gw60_applenvironmicrob_65_3_1099_s_319	0010049869	The observation that glutamate or glutamate-generating nitrogen substrates (arginine, proline, or histidine) repress GOGAT expression in  Salmonella typhimurium and  Klebsiella aerogenes during N-limited growth ( 6,  7) is in agreement with this hypothesis.	transcription
52581	2	334863	6	NULL	NULL	0	NULL	arginine	NULL		repress	NULL				GOGAT	NULL	expression of 			NULL	Salmonella typhimurium	0	NULL	NULL	NULL	gw60_applenvironmicrob_65_3_1099_s_319	0010049869	The observation that glutamate or glutamate-generating nitrogen substrates (arginine, proline, or histidine) repress GOGAT expression in  Salmonella typhimurium and  Klebsiella aerogenes during N-limited growth ( 6,  7) is in agreement with this hypothesis.	transcription
52582	3	334863	6	NULL	NULL	0	NULL	proline	NULL		repress	NULL				GOGAT	NULL	expression of 			NULL	Salmonella typhimurium	0	NULL	NULL	NULL	gw60_applenvironmicrob_65_3_1099_s_319	0010049869	The observation that glutamate or glutamate-generating nitrogen substrates (arginine, proline, or histidine) repress GOGAT expression in  Salmonella typhimurium and  Klebsiella aerogenes during N-limited growth ( 6,  7) is in agreement with this hypothesis.	transcription
52583	4	334863	6	NULL	NULL	0	NULL	histidine	NULL		repress	NULL				GOGAT	NULL	expression of 			NULL	Salmonella typhimurium	NULL	NULL	NULL	NULL	gw60_applenvironmicrob_65_3_1099_s_319	0010049869	The observation that glutamate or glutamate-generating nitrogen substrates (arginine, proline, or histidine) repress GOGAT expression in  Salmonella typhimurium and  Klebsiella aerogenes during N-limited growth ( 6,  7) is in agreement with this hypothesis.	transcription
52584	5	334863	6	NULL	NULL	0	NULL	arginine	NULL		is a type of 	NULL				glutamate-generating nitrogen substrate	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_3_1099_s_319	0010049869	The observation that glutamate or glutamate-generating nitrogen substrates (arginine, proline, or histidine) repress GOGAT expression in  Salmonella typhimurium and  Klebsiella aerogenes during N-limited growth ( 6,  7) is in agreement with this hypothesis.	transcription
52585	6	334863	6	NULL	NULL	0	NULL	proline	NULL		is a type of 	NULL				glutamate-generating nitrogen substrate	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_3_1099_s_319	0010049869	The observation that glutamate or glutamate-generating nitrogen substrates (arginine, proline, or histidine) repress GOGAT expression in  Salmonella typhimurium and  Klebsiella aerogenes during N-limited growth ( 6,  7) is in agreement with this hypothesis.	transcription
52586	7	334863	6	NULL	NULL	0	NULL	histidine	NULL		is a type of 	NULL				glutamate-generating nitrogen substrate	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_3_1099_s_319	0010049869	The observation that glutamate or glutamate-generating nitrogen substrates (arginine, proline, or histidine) repress GOGAT expression in  Salmonella typhimurium and  Klebsiella aerogenes during N-limited growth ( 6,  7) is in agreement with this hypothesis.	transcription
52587	8	334863	6	NULL	NULL	0	NULL	glutamate	NULL		repress	NULL				GOGAT	NULL	expression of 			NULL	Klebsiella aerogenes 	0	NULL	NULL	NULL	gw60_applenvironmicrob_65_3_1099_s_319	0010049869	The observation that glutamate or glutamate-generating nitrogen substrates (arginine, proline, or histidine) repress GOGAT expression in  Salmonella typhimurium and  Klebsiella aerogenes during N-limited growth ( 6,  7) is in agreement with this hypothesis.	transcription
52588	9	334863	6	NULL	NULL	0	NULL	arginine	NULL		repress	NULL				GOGAT	NULL	expression of 			NULL	Klebsiella aerogenes 	0	NULL	NULL	NULL	gw60_applenvironmicrob_65_3_1099_s_319	0010049869	The observation that glutamate or glutamate-generating nitrogen substrates (arginine, proline, or histidine) repress GOGAT expression in  Salmonella typhimurium and  Klebsiella aerogenes during N-limited growth ( 6,  7) is in agreement with this hypothesis.	transcription
52589	10	334863	6	NULL	NULL	0	NULL	proline	NULL		repress	NULL				GOGAT	NULL	expression of 			NULL	Klebsiella aerogenes 	0	NULL	NULL	NULL	gw60_applenvironmicrob_65_3_1099_s_319	0010049869	The observation that glutamate or glutamate-generating nitrogen substrates (arginine, proline, or histidine) repress GOGAT expression in  Salmonella typhimurium and  Klebsiella aerogenes during N-limited growth ( 6,  7) is in agreement with this hypothesis.	transcription
52590	11	334863	6	NULL	NULL	0	NULL	histidine	NULL		repress	NULL				GOGAT	NULL	expression of 			NULL	Klebsiella aerogenes 	0	NULL	NULL	NULL	gw60_applenvironmicrob_65_3_1099_s_319	0010049869	The observation that glutamate or glutamate-generating nitrogen substrates (arginine, proline, or histidine) repress GOGAT expression in  Salmonella typhimurium and  Klebsiella aerogenes during N-limited growth ( 6,  7) is in agreement with this hypothesis.	transcription
52591	1	334864	6	NULL	NULL	0	NULL		NULL	mutation of	causes	NULL		active site histidine		allosteric interactions	NULL	loss of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_18_17701_s_103	15749695	Since the active site histidine and glutamate mutations caused a loss of allosteric interactions, we tested whether the mutant enzymes could still be activated by ATP and triphosphate.	transcription
52592	2	334864	6	NULL	NULL	0	NULL		NULL	mutation of	causes	NULL		active site glutamate		allosteric interactions	NULL	loss of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_18_17701_s_103	15749695	Since the active site histidine and glutamate mutations caused a loss of allosteric interactions, we tested whether the mutant enzymes could still be activated by ATP and triphosphate.	transcription
51818	1	334865	5	NULL	NULL	0	NULL	histidine	NULL		activates	NULL				aspartate	NULL		Q701H		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_37_27471_s_281	16864587	For example, one could envision that the histidine activates the aspartate (Q701H) or the glutamate (double mutant) and therefore induces different levels of ATPase activity in a distance-dependent manner.	transcription
51819	2	334865	5	NULL	NULL	0	NULL	histidine	NULL		activates	NULL				glutamate	NULL	double mutant			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_37_27471_s_281	16864587	For example, one could envision that the histidine activates the aspartate (Q701H) or the glutamate (double mutant) and therefore induces different levels of ATPase activity in a distance-dependent manner.	transcription
51820	3	334865	5	NULL	NULL	0	NULL	statement 1	NULL		induce	NULL				ATPase activity	NULL	different levels of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_37_27471_s_281	16864587	For example, one could envision that the histidine activates the aspartate (Q701H) or the glutamate (double mutant) and therefore induces different levels of ATPase activity in a distance-dependent manner.	transcription
51821	4	334865	5	NULL	NULL	0	NULL	statement 2	NULL		induce	NULL				ATPase activity	NULL	different levels of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_37_27471_s_281	16864587	For example, one could envision that the histidine activates the aspartate (Q701H) or the glutamate (double mutant) and therefore induces different levels of ATPase activity in a distance-dependent manner.	transcription
52593	1	334865	6	NULL	NULL	0	NULL	histidine	NULL		activates	NULL					NULL		aspartate (Q701H)		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_37_27471_s_281	16864587	For example, one could envision that the histidine activates the aspartate (Q701H) or the glutamate (double mutant) and therefore induces different levels of ATPase activity in a distance-dependent manner.	transcription
52594	2	334865	6	NULL	NULL	0	NULL	histidine	NULL		activates	NULL					NULL		glutamate		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_37_27471_s_281	16864587	For example, one could envision that the histidine activates the aspartate (Q701H) or the glutamate (double mutant) and therefore induces different levels of ATPase activity in a distance-dependent manner.	transcription
52595	3	334865	6	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_37_27471_s_281	16864587	For example, one could envision that the histidine activates the aspartate (Q701H) or the glutamate (double mutant) and therefore induces different levels of ATPase activity in a distance-dependent manner.	transcription
52596	4	334865	6	NULL	NULL	0	NULL	statement 1	NULL		induces	NULL				ATPase 	NULL	activity of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_37_27471_s_281	16864587	For example, one could envision that the histidine activates the aspartate (Q701H) or the glutamate (double mutant) and therefore induces different levels of ATPase activity in a distance-dependent manner.	transcription
52597	5	334865	6	NULL	NULL	0	NULL	statement 2	NULL		induces	NULL				ATPase 	NULL	activity of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_37_27471_s_281	16864587	For example, one could envision that the histidine activates the aspartate (Q701H) or the glutamate (double mutant) and therefore induces different levels of ATPase activity in a distance-dependent manner.	transcription
51822	1	334866	5	NULL	NULL	0	NULL	cysteine	NULL		is an active site in	NULL				glutamine	NULL				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_13_7599_s_32	12799468	The active-site cysteine  covalently binds glutamine, and the histidine, initially protonated, donates a  proton to the amide group of glutamine to produce ammonia and glutamate.	transcription
51823	2	334866	5	NULL	NULL	0	NULL	glutamine	NULL		bind	NULL	covalently	cysteine		histidine	NULL	protonated			NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_13_7599_s_32	12799468	The active-site cysteine  covalently binds glutamine, and the histidine, initially protonated, donates a  proton to the amide group of glutamine to produce ammonia and glutamate.	transcription
51824	3	334866	5	NULL	NULL	0	NULL	histidine	NULL	protonated	donates	NULL				proton	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_100_13_7599_s_32	12799468	The active-site cysteine  covalently binds glutamine, and the histidine, initially protonated, donates a  proton to the amide group of glutamine to produce ammonia and glutamate.	transcription
51825	4	334866	5	NULL	NULL	0	NULL	proton	NULL		is donated to	NULL				glutamine	NULL		amide group		NULL		0	NULL	NULL	NULL	gw70_pnas_100_13_7599_s_32	12799468	The active-site cysteine  covalently binds glutamine, and the histidine, initially protonated, donates a  proton to the amide group of glutamine to produce ammonia and glutamate.	transcription
51826	5	334866	5	NULL	NULL	0	NULL	statement 4	NULL		produce	NULL				ammonia	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_100_13_7599_s_32	12799468	The active-site cysteine  covalently binds glutamine, and the histidine, initially protonated, donates a  proton to the amide group of glutamine to produce ammonia and glutamate.	transcription
51827	6	334866	5	NULL	NULL	0	NULL	statement 4	NULL		produce	NULL				glutamate	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_100_13_7599_s_32	12799468	The active-site cysteine  covalently binds glutamine, and the histidine, initially protonated, donates a  proton to the amide group of glutamine to produce ammonia and glutamate.	transcription
51828	7	334866	5	NULL	NULL	0	NULL	statement 5	NULL		occurs along with	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_100_13_7599_s_32	12799468	The active-site cysteine  covalently binds glutamine, and the histidine, initially protonated, donates a  proton to the amide group of glutamine to produce ammonia and glutamate.	transcription
52598	1	334866	6	NULL	NULL	0	NULL		NULL		bind	NULL	covalently	active-site cysteine		glutamine	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_100_13_7599_s_32	12799468	The active-site cysteine  covalently binds glutamine, and the histidine, initially protonated, donates a  proton to the amide group of glutamine to produce ammonia and glutamate.	transcription
52626	2	334866	6	NULL	NULL	0	NULL		NULL	protonated	donates 	NULL		histidine		proton	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_100_13_7599_s_32	12799468	The active-site cysteine  covalently binds glutamine, and the histidine, initially protonated, donates a  proton to the amide group of glutamine to produce ammonia and glutamate.	transcription
52627	3	334866	6	NULL	NULL	0	NULL	statement 2	NULL		occurs to	NULL				glutamine	NULL		amide group		NULL		0	NULL	NULL	NULL	gw70_pnas_100_13_7599_s_32	12799468	The active-site cysteine  covalently binds glutamine, and the histidine, initially protonated, donates a  proton to the amide group of glutamine to produce ammonia and glutamate.	transcription
52936	4	334866	6	NULL	NULL	0	NULL	statement 2	NULL		produce	NULL				ammonia	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_100_13_7599_s_32	12799468	The active-site cysteine  covalently binds glutamine, and the histidine, initially protonated, donates a  proton to the amide group of glutamine to produce ammonia and glutamate.	transcription
52937	5	334866	6	NULL	NULL	0	NULL	statement 2	NULL		produce	NULL				glutamate	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_100_13_7599_s_32	12799468	The active-site cysteine  covalently binds glutamine, and the histidine, initially protonated, donates a  proton to the amide group of glutamine to produce ammonia and glutamate.	transcription
51829	1	334867	5	NULL	NULL	0	NULL	Im gene	NULL		is homologous to	NULL				AOX	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_2_1190_s_30	11698414	The limited but significant homology of the  Im gene to the AOX includes several glutamate and histidine residues located in positions that could contribute to iron binding.	transcription
52628	1	334867	6	NULL	NULL	0	NULL	Im gene	NULL		is homologous to	NULL				AOX	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_2_1190_s_30	11698414	The limited but significant homology of the  Im gene to the AOX includes several glutamate and histidine residues located in positions that could contribute to iron binding.	transcription
51840	1	334868	5	NULL	NULL	0	NULL	Nt-FDH	NULL		is replaced with	NULL		histidine		Nt-FDH	NULL		alanine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_26_24030_s_8	11320079	Site-directed mutagenesis experiments showed that replacement of the histidine with alanine, asparagine, aspartate, glutamate, glutamine, or arginine in Nt-FDH resulted in expression of insoluble proteins.	transcription
51841	2	334868	5	NULL	NULL	0	NULL	statement 1	NULL		results in	NULL				insoluble proteins	NULL	expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_26_24030_s_8	11320079	Site-directed mutagenesis experiments showed that replacement of the histidine with alanine, asparagine, aspartate, glutamate, glutamine, or arginine in Nt-FDH resulted in expression of insoluble proteins.	transcription
51842	3	334868	5	NULL	NULL	0	NULL	Nt-FDH	NULL		is replaced with	NULL		histidine		Nt-FDH	NULL		asparagine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_26_24030_s_8	11320079	Site-directed mutagenesis experiments showed that replacement of the histidine with alanine, asparagine, aspartate, glutamate, glutamine, or arginine in Nt-FDH resulted in expression of insoluble proteins.	transcription
51843	4	334868	5	NULL	NULL	0	NULL	statement 3	NULL		results in	NULL				insoluble proteins	NULL	expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_26_24030_s_8	11320079	Site-directed mutagenesis experiments showed that replacement of the histidine with alanine, asparagine, aspartate, glutamate, glutamine, or arginine in Nt-FDH resulted in expression of insoluble proteins.	transcription
51844	5	334868	5	NULL	NULL	0	NULL	Nt-FDH	NULL		is replaced with	NULL		histidine		Nt-FDH	NULL		aspartate		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_26_24030_s_8	11320079	Site-directed mutagenesis experiments showed that replacement of the histidine with alanine, asparagine, aspartate, glutamate, glutamine, or arginine in Nt-FDH resulted in expression of insoluble proteins.	transcription
51845	6	334868	5	NULL	NULL	0	NULL	statement 5	NULL		results in	NULL				insoluble proteins	NULL	expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_26_24030_s_8	11320079	Site-directed mutagenesis experiments showed that replacement of the histidine with alanine, asparagine, aspartate, glutamate, glutamine, or arginine in Nt-FDH resulted in expression of insoluble proteins.	transcription
51846	7	334868	5	NULL	NULL	0	NULL	Nt-FDH	NULL		is replaced with	NULL		histidine		Nt-FDH	NULL		glutamate		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_26_24030_s_8	11320079	Site-directed mutagenesis experiments showed that replacement of the histidine with alanine, asparagine, aspartate, glutamate, glutamine, or arginine in Nt-FDH resulted in expression of insoluble proteins.	transcription
51847	8	334868	5	NULL	NULL	0	NULL	statement 7	NULL		results in	NULL				insoluble proteins	NULL	expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_26_24030_s_8	11320079	Site-directed mutagenesis experiments showed that replacement of the histidine with alanine, asparagine, aspartate, glutamate, glutamine, or arginine in Nt-FDH resulted in expression of insoluble proteins.	transcription
51848	9	334868	5	NULL	NULL	0	NULL	Nt-FDH	NULL		is replaced with	NULL		histidine		Nt-FDH	NULL		glutamine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_26_24030_s_8	11320079	Site-directed mutagenesis experiments showed that replacement of the histidine with alanine, asparagine, aspartate, glutamate, glutamine, or arginine in Nt-FDH resulted in expression of insoluble proteins.	transcription
51849	10	334868	5	NULL	NULL	0	NULL	statement 9	NULL		results in	NULL				insoluble proteins	NULL	expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_26_24030_s_8	11320079	Site-directed mutagenesis experiments showed that replacement of the histidine with alanine, asparagine, aspartate, glutamate, glutamine, or arginine in Nt-FDH resulted in expression of insoluble proteins.	transcription
51850	11	334868	5	NULL	NULL	0	NULL	Nt-FDH	NULL		is replaced with	NULL		histidine		Nt-FDH	NULL		arginine 		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_26_24030_s_8	11320079	Site-directed mutagenesis experiments showed that replacement of the histidine with alanine, asparagine, aspartate, glutamate, glutamine, or arginine in Nt-FDH resulted in expression of insoluble proteins.	transcription
51851	12	334868	5	NULL	NULL	0	NULL	statement 11	NULL		results in	NULL				insoluble proteins	NULL	expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_26_24030_s_8	11320079	Site-directed mutagenesis experiments showed that replacement of the histidine with alanine, asparagine, aspartate, glutamate, glutamine, or arginine in Nt-FDH resulted in expression of insoluble proteins.	transcription
51830	1	334869	5	NULL	NULL	0	NULL	GLYT1b	NULL		is homologous to	NULL				DAT	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_22_22983_s_120	15031290	Based on the homology between GLYT1b and DAT, we targeted histidine residues and a select number of glutamate residues, which are predicted to be on the extracellular domains of GLYT1b and in similar locations to the Zn2+-binding residues of DAT.	transcription
52465	1	334870	5	NULL	NULL	0	NULL	xylose	NULL		interacts with	NULL		O-2		asparagine	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_10_9597_s_24	14668328	The data show that at the -1 subsite the O-3 of xylose makes a hydrogen bond with a highly conserved lysine and histidine, whereas O-2 interacts with an asparagine and a glutamate (which acts as the catalytic nucleophile) that are invariant in GH10 xylanases.	transcription
52466	2	334870	5	NULL	NULL	0	NULL	xylose	NULL		interacts with	NULL		O-2		glutamate	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_10_9597_s_24	14668328	The data show that at the -1 subsite the O-3 of xylose makes a hydrogen bond with a highly conserved lysine and histidine, whereas O-2 interacts with an asparagine and a glutamate (which acts as the catalytic nucleophile) that are invariant in GH10 xylanases.	transcription
52467	3	334870	5	NULL	NULL	0	NULL	glutamate	NULL		acts as	NULL				catalytic nucleophile	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_10_9597_s_24	14668328	The data show that at the -1 subsite the O-3 of xylose makes a hydrogen bond with a highly conserved lysine and histidine, whereas O-2 interacts with an asparagine and a glutamate (which acts as the catalytic nucleophile) that are invariant in GH10 xylanases.	transcription
52522	4	334870	5	NULL	NULL	0	NULL	xylose	NULL		hydrogen-bonds with	NULL		O-3		lysine	NULL	highly conserved			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_10_9597_s_24	14668328	The data show that at the -1 subsite the O-3 of xylose makes a hydrogen bond with a highly conserved lysine and histidine, whereas O-2 interacts with an asparagine and a glutamate (which acts as the catalytic nucleophile) that are invariant in GH10 xylanases.	transcription
52523	5	334870	5	NULL	NULL	0	NULL	xylose	NULL		hydrogen-bonds with	NULL		O-3		histidine	NULL	highly conserved			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_10_9597_s_24	14668328	The data show that at the -1 subsite the O-3 of xylose makes a hydrogen bond with a highly conserved lysine and histidine, whereas O-2 interacts with an asparagine and a glutamate (which acts as the catalytic nucleophile) that are invariant in GH10 xylanases.	transcription
52629	1	334870	6	NULL	NULL	0	NULL	xylose	NULL		bind	NULL		1 subsite the O-3		lysine 	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_10_9597_s_24	14668328	The data show that at the -1 subsite the O-3 of xylose makes a hydrogen bond with a highly conserved lysine and histidine, whereas O-2 interacts with an asparagine and a glutamate (which acts as the catalytic nucleophile) that are invariant in GH10 xylanases.	transcription
52630	2	334870	6	NULL	NULL	0	NULL	xylose	NULL		bind	NULL		1 subsite the O-3		histidine	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_10_9597_s_24	14668328	The data show that at the -1 subsite the O-3 of xylose makes a hydrogen bond with a highly conserved lysine and histidine, whereas O-2 interacts with an asparagine and a glutamate (which acts as the catalytic nucleophile) that are invariant in GH10 xylanases.	transcription
52631	3	334870	6	NULL	NULL	0	NULL	O-2	NULL		interacts with	NULL				asparagine	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_10_9597_s_24	14668328	The data show that at the -1 subsite the O-3 of xylose makes a hydrogen bond with a highly conserved lysine and histidine, whereas O-2 interacts with an asparagine and a glutamate (which acts as the catalytic nucleophile) that are invariant in GH10 xylanases.	transcription
52632	4	334870	6	NULL	NULL	0	NULL	O-2	NULL		interacts with	NULL				glutamate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_10_9597_s_24	14668328	The data show that at the -1 subsite the O-3 of xylose makes a hydrogen bond with a highly conserved lysine and histidine, whereas O-2 interacts with an asparagine and a glutamate (which acts as the catalytic nucleophile) that are invariant in GH10 xylanases.	transcription
52633	1	334871	6	NULL	NULL	0	NULL		NULL		does not show	NULL		D668E		ATPase activity	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_37_27471_s_54	16864587	Although the D668E mutant like the wild-type enzyme did not show ATPase activity, reintroduction of the histidine in the absence of the glutamate (Q701H) resulted in an ATPase-active enzyme, although at a reduced level compared with the double mutant (D668E/Q701H).	transcription
52634	2	334871	6	NULL	NULL	0	NULL		NULL		shows	NULL		Q701H		ATPase activity	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_37_27471_s_54	16864587	Although the D668E mutant like the wild-type enzyme did not show ATPase activity, reintroduction of the histidine in the absence of the glutamate (Q701H) resulted in an ATPase-active enzyme, although at a reduced level compared with the double mutant (D668E/Q701H).	transcription
52635	3	334871	6	NULL	NULL	0	NULL		NULL		shows	NULL		D668E/Q701H		ATPase activity	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_37_27471_s_54	16864587	Although the D668E mutant like the wild-type enzyme did not show ATPase activity, reintroduction of the histidine in the absence of the glutamate (Q701H) resulted in an ATPase-active enzyme, although at a reduced level compared with the double mutant (D668E/Q701H).	transcription
52636	4	334871	6	NULL	NULL	0	NULL	statement 2	NULL		is reduced as compared to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_37_27471_s_54	16864587	Although the D668E mutant like the wild-type enzyme did not show ATPase activity, reintroduction of the histidine in the absence of the glutamate (Q701H) resulted in an ATPase-active enzyme, although at a reduced level compared with the double mutant (D668E/Q701H).	transcription
51852	1	334872	5	NULL	NULL	0	NULL	fumarylacetoacetate hydrolase	NULL		is composed of	NULL		active site		catalytic triad	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_50_50091_s_233	14506266	As described in detail by Timm and co-workers ( ,  ), the active site of fumarylacetoacetate hydrolase is composed of a catalytic triad consisting of a glutamate carboxylate that stabilizes a histidine base that directly activates a nucleophilic water molecule.	transcription
51853	2	334872	5	NULL	NULL	0	NULL	catalytic triad	NULL		consists of	NULL				glutamate carboxylate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_50_50091_s_233	14506266	As described in detail by Timm and co-workers ( ,  ), the active site of fumarylacetoacetate hydrolase is composed of a catalytic triad consisting of a glutamate carboxylate that stabilizes a histidine base that directly activates a nucleophilic water molecule.	transcription
51854	3	334872	5	NULL	NULL	0	NULL	glutamate carboxylate	NULL		stabilize	NULL				histidine base	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_50_50091_s_233	14506266	As described in detail by Timm and co-workers ( ,  ), the active site of fumarylacetoacetate hydrolase is composed of a catalytic triad consisting of a glutamate carboxylate that stabilizes a histidine base that directly activates a nucleophilic water molecule.	transcription
51855	4	334872	5	NULL	NULL	0	NULL	histidine base	NULL		activates	NULL	directly			water molecule	NULL	nucleophilic			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_50_50091_s_233	14506266	As described in detail by Timm and co-workers ( ,  ), the active site of fumarylacetoacetate hydrolase is composed of a catalytic triad consisting of a glutamate carboxylate that stabilizes a histidine base that directly activates a nucleophilic water molecule.	transcription
52973	1	334872	6	NULL	NULL	0	NULL	fumarylacetoacetate hydrolase	NULL		is composed of	NULL		active site		catalytic triad	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_50_50091_s_233	14506266	As described in detail by Timm and co-workers ( ,  ), the active site of fumarylacetoacetate hydrolase is composed of a catalytic triad consisting of a glutamate carboxylate that stabilizes a histidine base that directly activates a nucleophilic water molecule.	transcription
52974	2	334872	6	NULL	NULL	0	NULL	catalytic site 	NULL		consists of	NULL				glutamate carboxylate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_50_50091_s_233	14506266	As described in detail by Timm and co-workers ( ,  ), the active site of fumarylacetoacetate hydrolase is composed of a catalytic triad consisting of a glutamate carboxylate that stabilizes a histidine base that directly activates a nucleophilic water molecule.	transcription
52975	3	334872	6	NULL	NULL	0	NULL	glutamate carboxylate	NULL		stabilize	NULL				histidine base	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_50_50091_s_233	14506266	As described in detail by Timm and co-workers ( ,  ), the active site of fumarylacetoacetate hydrolase is composed of a catalytic triad consisting of a glutamate carboxylate that stabilizes a histidine base that directly activates a nucleophilic water molecule.	transcription
52976	4	334872	6	NULL	NULL	0	NULL	histidine base	NULL		activates	NULL	directly			water molecule	NULL	nucleophilic			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_50_50091_s_233	14506266	As described in detail by Timm and co-workers ( ,  ), the active site of fumarylacetoacetate hydrolase is composed of a catalytic triad consisting of a glutamate carboxylate that stabilizes a histidine base that directly activates a nucleophilic water molecule.	transcription
51856	1	334876	5	NULL	NULL	0	NULL	AHR	NULL		bind	NULL		glutamate;;arginine;;histidine		DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_49_31657_s_229	8940186	We have demonstrated that the amino acids involved in DNA binding of the AHR and ARNT, glutamate, arginine, and histidine residues, are similar to those involved in amino acid/nucleotide interactions of other bHLH proteins.	transcription
51857	2	334876	5	NULL	NULL	0	NULL	ARNT	NULL		bind	NULL		glutamate;;arginine;;histidine		DNA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_49_31657_s_229	8940186	We have demonstrated that the amino acids involved in DNA binding of the AHR and ARNT, glutamate, arginine, and histidine residues, are similar to those involved in amino acid/nucleotide interactions of other bHLH proteins.	transcription
52637	1	334876	6	NULL	NULL	0	NULL	DNA	NULL		bind	NULL				AHR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_49_31657_s_229	8940186	We have demonstrated that the amino acids involved in DNA binding of the AHR and ARNT, glutamate, arginine, and histidine residues, are similar to those involved in amino acid/nucleotide interactions of other bHLH proteins.	transcription
52638	2	334876	6	NULL	NULL	0	NULL	DNA	NULL		bind	NULL				ARNT	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_49_31657_s_229	8940186	We have demonstrated that the amino acids involved in DNA binding of the AHR and ARNT, glutamate, arginine, and histidine residues, are similar to those involved in amino acid/nucleotide interactions of other bHLH proteins.	transcription
52506	1	334877	5	NULL	NULL	0	NULL	PH1704	NULL		is similar to	NULL		catalytic triad		papain type cysteine proteases	NULL		triads		NULL		0	NULL	NULL	NULL	gw60_pnas_97_26_14079_s_144	11114201	The catalytic triad in PH1704 shares the same handedness with the triads in papain type cysteine proteases, namely the cysteine interacts with deltaN, whereas the glutamate hydrogen-bonds with  N of the histidine (Fig.  4 D).	transcription
52507	2	334877	5	NULL	NULL	0	NULL	cysteine	NULL		interacts with	NULL					NULL		deltaN		NULL		0	NULL	NULL	NULL	gw60_pnas_97_26_14079_s_144	11114201	The catalytic triad in PH1704 shares the same handedness with the triads in papain type cysteine proteases, namely the cysteine interacts with deltaN, whereas the glutamate hydrogen-bonds with  N of the histidine (Fig.  4 D).	transcription
52508	3	334877	5	NULL	NULL	0	NULL	glutamate	NULL		hydrogen-bonds with	NULL				histidine	NULL		N		NULL		0	NULL	NULL	NULL	gw60_pnas_97_26_14079_s_144	11114201	The catalytic triad in PH1704 shares the same handedness with the triads in papain type cysteine proteases, namely the cysteine interacts with deltaN, whereas the glutamate hydrogen-bonds with  N of the histidine (Fig.  4 D).	transcription
52639	1	334877	6	NULL	NULL	0	NULL	cysteine	NULL		interacts with	NULL				deltaN	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_97_26_14079_s_144	11114201	The catalytic triad in PH1704 shares the same handedness with the triads in papain type cysteine proteases, namely the cysteine interacts with deltaN, whereas the glutamate hydrogen-bonds with  N of the histidine (Fig.  4 D).	transcription
52640	2	334877	6	NULL	NULL	0	NULL		NULL		bind	NULL		glutamate hydrogen			NULL		N of histidine		NULL		0	NULL	NULL	NULL	gw60_pnas_97_26_14079_s_144	11114201	The catalytic triad in PH1704 shares the same handedness with the triads in papain type cysteine proteases, namely the cysteine interacts with deltaN, whereas the glutamate hydrogen-bonds with  N of the histidine (Fig.  4 D).	transcription
52509	1	334878	5	NULL	NULL	0	NULL	alanine	NULL		inhibit	NULL	strongly			glutamine	NULL	transport of			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_93	15581847	As shown in   Table 1, alanine, serine, threonine, cysteine, asparagine, methionine and valine strongly  inhibited the glutamine transport; the inhibition by these amino acids ranged from  54% to 70% at 1 mM and was virtually complete at a concentration of 10 mM. Glycine,  proline, arginine, histidine, glutamate and creatine had a low inhibitory effect.	transcription
52510	2	334878	5	NULL	NULL	0	NULL	serine	NULL		inhibit	NULL	strongly			glutamine	NULL	transport of			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_93	15581847	As shown in   Table 1, alanine, serine, threonine, cysteine, asparagine, methionine and valine strongly  inhibited the glutamine transport; the inhibition by these amino acids ranged from  54% to 70% at 1 mM and was virtually complete at a concentration of 10 mM. Glycine,  proline, arginine, histidine, glutamate and creatine had a low inhibitory effect.	transcription
52511	3	334878	5	NULL	NULL	0	NULL	threonine	NULL		inhibit	NULL	strongly			glutamine	NULL	transport of			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_93	15581847	As shown in   Table 1, alanine, serine, threonine, cysteine, asparagine, methionine and valine strongly  inhibited the glutamine transport; the inhibition by these amino acids ranged from  54% to 70% at 1 mM and was virtually complete at a concentration of 10 mM. Glycine,  proline, arginine, histidine, glutamate and creatine had a low inhibitory effect.	transcription
52512	4	334878	5	NULL	NULL	0	NULL	cysteine	NULL		inhibit	NULL	strongly			glutamine	NULL	transport of			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_93	15581847	As shown in   Table 1, alanine, serine, threonine, cysteine, asparagine, methionine and valine strongly  inhibited the glutamine transport; the inhibition by these amino acids ranged from  54% to 70% at 1 mM and was virtually complete at a concentration of 10 mM. Glycine,  proline, arginine, histidine, glutamate and creatine had a low inhibitory effect.	transcription
52513	5	334878	5	NULL	NULL	0	NULL	asparagine	NULL		inhibit	NULL	strongly			glutamine	NULL	transport of			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_93	15581847	As shown in   Table 1, alanine, serine, threonine, cysteine, asparagine, methionine and valine strongly  inhibited the glutamine transport; the inhibition by these amino acids ranged from  54% to 70% at 1 mM and was virtually complete at a concentration of 10 mM. Glycine,  proline, arginine, histidine, glutamate and creatine had a low inhibitory effect.	transcription
52514	6	334878	5	NULL	NULL	0	NULL	methionine	NULL		inhibit	NULL	strongly			glutamine	NULL	transport of			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_93	15581847	As shown in   Table 1, alanine, serine, threonine, cysteine, asparagine, methionine and valine strongly  inhibited the glutamine transport; the inhibition by these amino acids ranged from  54% to 70% at 1 mM and was virtually complete at a concentration of 10 mM. Glycine,  proline, arginine, histidine, glutamate and creatine had a low inhibitory effect.	transcription
52515	7	334878	5	NULL	NULL	0	NULL	valine	NULL		inhibit	NULL	strongly			glutamine	NULL	transport of			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_93	15581847	As shown in   Table 1, alanine, serine, threonine, cysteine, asparagine, methionine and valine strongly  inhibited the glutamine transport; the inhibition by these amino acids ranged from  54% to 70% at 1 mM and was virtually complete at a concentration of 10 mM. Glycine,  proline, arginine, histidine, glutamate and creatine had a low inhibitory effect.	transcription
52516	8	334878	5	NULL	NULL	0	NULL	glycine	NULL		inhibit	NULL				glutamine	NULL	transport of			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_93	15581847	As shown in   Table 1, alanine, serine, threonine, cysteine, asparagine, methionine and valine strongly  inhibited the glutamine transport; the inhibition by these amino acids ranged from  54% to 70% at 1 mM and was virtually complete at a concentration of 10 mM. Glycine,  proline, arginine, histidine, glutamate and creatine had a low inhibitory effect.	transcription
52517	9	334878	5	NULL	NULL	0	NULL	proline	NULL		inhibit	NULL				glutamine	NULL	transport of			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_93	15581847	As shown in   Table 1, alanine, serine, threonine, cysteine, asparagine, methionine and valine strongly  inhibited the glutamine transport; the inhibition by these amino acids ranged from  54% to 70% at 1 mM and was virtually complete at a concentration of 10 mM. Glycine,  proline, arginine, histidine, glutamate and creatine had a low inhibitory effect.	transcription
52518	10	334878	5	NULL	NULL	0	NULL	arginine	NULL		inhibit	NULL				glutamine	NULL	transport of			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_93	15581847	As shown in   Table 1, alanine, serine, threonine, cysteine, asparagine, methionine and valine strongly  inhibited the glutamine transport; the inhibition by these amino acids ranged from  54% to 70% at 1 mM and was virtually complete at a concentration of 10 mM. Glycine,  proline, arginine, histidine, glutamate and creatine had a low inhibitory effect.	transcription
52519	11	334878	5	NULL	NULL	0	NULL	histidine	NULL		inhibit	NULL				glutamine	NULL	transport of			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_93	15581847	As shown in   Table 1, alanine, serine, threonine, cysteine, asparagine, methionine and valine strongly  inhibited the glutamine transport; the inhibition by these amino acids ranged from  54% to 70% at 1 mM and was virtually complete at a concentration of 10 mM. Glycine,  proline, arginine, histidine, glutamate and creatine had a low inhibitory effect.	transcription
52520	12	334878	5	NULL	NULL	0	NULL	glutamate	NULL		inhibit	NULL				glutamine	NULL	transport of			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_93	15581847	As shown in   Table 1, alanine, serine, threonine, cysteine, asparagine, methionine and valine strongly  inhibited the glutamine transport; the inhibition by these amino acids ranged from  54% to 70% at 1 mM and was virtually complete at a concentration of 10 mM. Glycine,  proline, arginine, histidine, glutamate and creatine had a low inhibitory effect.	transcription
52521	13	334878	5	NULL	NULL	0	NULL	creatine	NULL		inhibit	NULL				glutamine	NULL	transport of			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_93	15581847	As shown in   Table 1, alanine, serine, threonine, cysteine, asparagine, methionine and valine strongly  inhibited the glutamine transport; the inhibition by these amino acids ranged from  54% to 70% at 1 mM and was virtually complete at a concentration of 10 mM. Glycine,  proline, arginine, histidine, glutamate and creatine had a low inhibitory effect.	transcription
52641	1	334878	6	NULL	NULL	0	NULL	alanine	NULL		inhibits	NULL	strongly			glutamine	NULL	transport of 			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_93	15581847	As shown in   Table 1, alanine, serine, threonine, cysteine, asparagine, methionine and valine strongly  inhibited the glutamine transport; the inhibition by these amino acids ranged from  54% to 70% at 1 mM and was virtually complete at a concentration of 10 mM. Glycine,  proline, arginine, histidine, glutamate and creatine had a low inhibitory effect.	transcription
52642	2	334878	6	NULL	NULL	0	NULL	serine	NULL		inhibits	NULL	strongly			glutamine	NULL	transport of 			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_93	15581847	As shown in   Table 1, alanine, serine, threonine, cysteine, asparagine, methionine and valine strongly  inhibited the glutamine transport; the inhibition by these amino acids ranged from  54% to 70% at 1 mM and was virtually complete at a concentration of 10 mM. Glycine,  proline, arginine, histidine, glutamate and creatine had a low inhibitory effect.	transcription
52643	3	334878	6	NULL	NULL	0	NULL	threonine	NULL		inhibits	NULL	strongly			glutamine	NULL	transport of 			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_93	15581847	As shown in   Table 1, alanine, serine, threonine, cysteine, asparagine, methionine and valine strongly  inhibited the glutamine transport; the inhibition by these amino acids ranged from  54% to 70% at 1 mM and was virtually complete at a concentration of 10 mM. Glycine,  proline, arginine, histidine, glutamate and creatine had a low inhibitory effect.	transcription
52644	4	334878	6	NULL	NULL	0	NULL	cysteine	NULL		inhibits	NULL	strongly			glutamine	NULL	transport of 			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_93	15581847	As shown in   Table 1, alanine, serine, threonine, cysteine, asparagine, methionine and valine strongly  inhibited the glutamine transport; the inhibition by these amino acids ranged from  54% to 70% at 1 mM and was virtually complete at a concentration of 10 mM. Glycine,  proline, arginine, histidine, glutamate and creatine had a low inhibitory effect.	transcription
52645	5	334878	6	NULL	NULL	0	NULL	asparagine	NULL		inhibits	NULL	strongly			glutamine	NULL	transport of 			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_93	15581847	As shown in   Table 1, alanine, serine, threonine, cysteine, asparagine, methionine and valine strongly  inhibited the glutamine transport; the inhibition by these amino acids ranged from  54% to 70% at 1 mM and was virtually complete at a concentration of 10 mM. Glycine,  proline, arginine, histidine, glutamate and creatine had a low inhibitory effect.	transcription
52646	6	334878	6	NULL	NULL	0	NULL	methionine	NULL		inhibits	NULL	strongly			glutamine	NULL	transport of 			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_93	15581847	As shown in   Table 1, alanine, serine, threonine, cysteine, asparagine, methionine and valine strongly  inhibited the glutamine transport; the inhibition by these amino acids ranged from  54% to 70% at 1 mM and was virtually complete at a concentration of 10 mM. Glycine,  proline, arginine, histidine, glutamate and creatine had a low inhibitory effect.	transcription
52647	7	334878	6	NULL	NULL	0	NULL	valine	NULL		inhibits	NULL	strongly			glutamine	NULL	transport of 			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_93	15581847	As shown in   Table 1, alanine, serine, threonine, cysteine, asparagine, methionine and valine strongly  inhibited the glutamine transport; the inhibition by these amino acids ranged from  54% to 70% at 1 mM and was virtually complete at a concentration of 10 mM. Glycine,  proline, arginine, histidine, glutamate and creatine had a low inhibitory effect.	transcription
52648	8	334878	6	NULL	NULL	0	NULL	glycine	NULL		inhibits	NULL	weakly			glutamine	NULL	transport of 			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_93	15581847	As shown in   Table 1, alanine, serine, threonine, cysteine, asparagine, methionine and valine strongly  inhibited the glutamine transport; the inhibition by these amino acids ranged from  54% to 70% at 1 mM and was virtually complete at a concentration of 10 mM. Glycine,  proline, arginine, histidine, glutamate and creatine had a low inhibitory effect.	transcription
52649	9	334878	6	NULL	NULL	0	NULL	proline	NULL		inhibits	NULL	weakly			glutamine	NULL	transport of 			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_93	15581847	As shown in   Table 1, alanine, serine, threonine, cysteine, asparagine, methionine and valine strongly  inhibited the glutamine transport; the inhibition by these amino acids ranged from  54% to 70% at 1 mM and was virtually complete at a concentration of 10 mM. Glycine,  proline, arginine, histidine, glutamate and creatine had a low inhibitory effect.	transcription
52650	10	334878	6	NULL	NULL	0	NULL	arginine	NULL		inhibits	NULL	weakly			glutamine	NULL	transport of 			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_93	15581847	As shown in   Table 1, alanine, serine, threonine, cysteine, asparagine, methionine and valine strongly  inhibited the glutamine transport; the inhibition by these amino acids ranged from  54% to 70% at 1 mM and was virtually complete at a concentration of 10 mM. Glycine,  proline, arginine, histidine, glutamate and creatine had a low inhibitory effect.	transcription
52651	11	334878	6	NULL	NULL	0	NULL	histidine	NULL		inhibits	NULL	weakly			glutamine	NULL	transport of 			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_93	15581847	As shown in   Table 1, alanine, serine, threonine, cysteine, asparagine, methionine and valine strongly  inhibited the glutamine transport; the inhibition by these amino acids ranged from  54% to 70% at 1 mM and was virtually complete at a concentration of 10 mM. Glycine,  proline, arginine, histidine, glutamate and creatine had a low inhibitory effect.	transcription
52652	12	334878	6	NULL	NULL	0	NULL	glutamate	NULL		inhibits	NULL	weakly			glutamine	NULL	transport of 			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_93	15581847	As shown in   Table 1, alanine, serine, threonine, cysteine, asparagine, methionine and valine strongly  inhibited the glutamine transport; the inhibition by these amino acids ranged from  54% to 70% at 1 mM and was virtually complete at a concentration of 10 mM. Glycine,  proline, arginine, histidine, glutamate and creatine had a low inhibitory effect.	transcription
52653	13	334878	6	NULL	NULL	0	NULL	creatine	NULL		inhibits	NULL	weakly			glutamine	NULL	transport of 			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_93	15581847	As shown in   Table 1, alanine, serine, threonine, cysteine, asparagine, methionine and valine strongly  inhibited the glutamine transport; the inhibition by these amino acids ranged from  54% to 70% at 1 mM and was virtually complete at a concentration of 10 mM. Glycine,  proline, arginine, histidine, glutamate and creatine had a low inhibitory effect.	transcription
51858	1	334879	5	NULL	NULL	0	NULL	pgiA	NULL		corresponds to	NULL		His311			NULL		active-site histidine		NULL		0	NULL	NULL	NULL	gw60_febslett_499_1_11_s_132	11418102	According to the binding position of the inhibitor, they proposed a different mechanism in which the active-site histidine and lysine (corresponding to His311 and Lys425 of pgiA) catalyze the opening of the cyclic form substrates, and the active-site glutamate (corresponding to Glu290 of pgiA) takes the responsibility for the isomerization.	transcription
51859	2	334879	5	NULL	NULL	0	NULL	pgiA	NULL		corresponds to	NULL		Lys425			NULL		active-site lysine		NULL		0	NULL	NULL	NULL	gw60_febslett_499_1_11_s_132	11418102	According to the binding position of the inhibitor, they proposed a different mechanism in which the active-site histidine and lysine (corresponding to His311 and Lys425 of pgiA) catalyze the opening of the cyclic form substrates, and the active-site glutamate (corresponding to Glu290 of pgiA) takes the responsibility for the isomerization.	transcription
51860	3	334879	5	NULL	NULL	0	NULL	statement 1	NULL		catalyze	NULL				cyclic form substrates	NULL	opening of			NULL		0	NULL	NULL	NULL	gw60_febslett_499_1_11_s_132	11418102	According to the binding position of the inhibitor, they proposed a different mechanism in which the active-site histidine and lysine (corresponding to His311 and Lys425 of pgiA) catalyze the opening of the cyclic form substrates, and the active-site glutamate (corresponding to Glu290 of pgiA) takes the responsibility for the isomerization.	transcription
51861	4	334879	5	NULL	NULL	0	NULL	statement 1	NULL		catalyze	NULL				cyclic form substrates	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_499_1_11_s_132	11418102	According to the binding position of the inhibitor, they proposed a different mechanism in which the active-site histidine and lysine (corresponding to His311 and Lys425 of pgiA) catalyze the opening of the cyclic form substrates, and the active-site glutamate (corresponding to Glu290 of pgiA) takes the responsibility for the isomerization.	transcription
51862	5	334879	5	NULL	NULL	0	NULL	pgiA	NULL		corresponds to	NULL		Glu290			NULL		active-site glutamate		NULL		0	NULL	NULL	NULL	gw60_febslett_499_1_11_s_132	11418102	According to the binding position of the inhibitor, they proposed a different mechanism in which the active-site histidine and lysine (corresponding to His311 and Lys425 of pgiA) catalyze the opening of the cyclic form substrates, and the active-site glutamate (corresponding to Glu290 of pgiA) takes the responsibility for the isomerization.	transcription
51863	6	334879	5	NULL	NULL	0	NULL	statement 5	NULL		is responsible for	NULL				isomerization	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_499_1_11_s_132	11418102	According to the binding position of the inhibitor, they proposed a different mechanism in which the active-site histidine and lysine (corresponding to His311 and Lys425 of pgiA) catalyze the opening of the cyclic form substrates, and the active-site glutamate (corresponding to Glu290 of pgiA) takes the responsibility for the isomerization.	transcription
51864	1	334880	5	NULL	NULL	0	NULL	methylisocitrate lyase	NULL		is important for	NULL		[KR-C-G-H[LMQR]		methylisocitrate lyase	NULL	catalytic activity of			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_1_271_s_126	11772636	[KR-C-G-H[LMQR]) was present, as it is in all known methylisocitrate lyase sequences; this signature includes highly conserved cysteine (C), glutamate (G), and histidine (H) residues which are important for the catalytic activity of isocitrate lyases ( http://www.expasy.	transcription
53713	1	334880	6	NULL	NULL	0	NULL	isocitrate lyases			exhibits					catalytic activity					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_1_271_s_126	11772636	[KR-C-G-H[LMQR]) was present, as it is in all known methylisocitrate lyase sequences; this signature includes highly conserved cysteine (C), glutamate (G), and histidine (H) residues which are important for the catalytic activity of isocitrate lyases ( http://www.expasy.	transcription
53715	2	334880	6	NULL	NULL	0	NULL				is important for			[KR-C-G-H[LMQR]		statement 1					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_1_271_s_126	11772636	[KR-C-G-H[LMQR]) was present, as it is in all known methylisocitrate lyase sequences; this signature includes highly conserved cysteine (C), glutamate (G), and histidine (H) residues which are important for the catalytic activity of isocitrate lyases ( http://www.expasy.	transcription
51865	1	334881	5	NULL	NULL	0	NULL	NixA	NULL		bind	NULL		histidine;;aspartate;;glutamate		nickel	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_jbacteriol_184_5_1438_s_36	11844775	In two previous papers, the consequences of amino acid replacements in high-affinity nickel transporters were studied: one concentrated on the conserved motif in TM II of the NixA homologue HoxN ( 7), and the other focused on conserved histidine, aspartate, and glutamate residues of NixA ( 12), well known to bind nickel in vitro.	transcription
52654	1	334881	6	NULL	NULL	0	NULL	NixA	NULL		bind	NULL				nickel	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw60_jbacteriol_184_5_1438_s_36	11844775	In two previous papers, the consequences of amino acid replacements in high-affinity nickel transporters were studied: one concentrated on the conserved motif in TM II of the NixA homologue HoxN ( 7), and the other focused on conserved histidine, aspartate, and glutamate residues of NixA ( 12), well known to bind nickel in vitro.	transcription
51866	1	334882	5	NULL	NULL	0	NULL		NULL	protonation of	is mediated by	NULL		Calpha			NULL		histidine residue		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_4_1939_s_163	9442028	An earlier study of the effects of D2O on the reaction catalyzed by glutamate decarboxylase has already shown large solvent isotope effects ( 25) and these have been cited in support of a proposal that, after the decarboxylation step, protonation at Calpha is mediated by a histidine residue ( 16).	transcription
51867	2	334882	5	NULL	NULL	0	NULL	statement 1	NULL		occurs after	NULL				decarboxylation step	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_4_1939_s_163	9442028	An earlier study of the effects of D2O on the reaction catalyzed by glutamate decarboxylase has already shown large solvent isotope effects ( 25) and these have been cited in support of a proposal that, after the decarboxylation step, protonation at Calpha is mediated by a histidine residue ( 16).	transcription
52800	1	334882	6	NULL	NULL	0	NULL	Calpha	NULL	protonation at	is mediated by	NULL					NULL		histidine residue		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_4_1939_s_163	9442028	An earlier study of the effects of D2O on the reaction catalyzed by glutamate decarboxylase has already shown large solvent isotope effects ( 25) and these have been cited in support of a proposal that, after the decarboxylation step, protonation at Calpha is mediated by a histidine residue ( 16).	transcription
52801	2	334882	6	NULL	NULL	0	NULL	statement 1	NULL		occurs after	NULL				decarboxylation step	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_4_1939_s_163	9442028	An earlier study of the effects of D2O on the reaction catalyzed by glutamate decarboxylase has already shown large solvent isotope effects ( 25) and these have been cited in support of a proposal that, after the decarboxylation step, protonation at Calpha is mediated by a histidine residue ( 16).	transcription
54306	1	334883	5	NULL	NULL	0	NULL	histidine			is a substrate for			E2-157		arginine			E2-157		NULL	newborn CD-1 mice	NULL	NULL	NULL	NULL	abs-batch0620-0649_virology_347_1_16380143_s_4	16380143	However, substitution of histidine  for arginine at E2-157 (R157H) or glutamate for lysine at E2-159 (K159E)  produces viruses with decreases in heparin-Sepharose binding and increases  in viremia but different levels of binding to HS-expressing cells and  virulence phenotypes in newborn CD-1 mice (Byrnes, A.P., Griffin, D.E.,  2000.	transcription
54307	2	334883	5	NULL	NULL	0	NULL	glutamate			is a substrate for			E2-159		lysine			E2-159		NULL	newborn CD-1 mice	0	NULL	NULL	NULL	abs-batch0620-0649_virology_347_1_16380143_s_4	16380143	However, substitution of histidine  for arginine at E2-157 (R157H) or glutamate for lysine at E2-159 (K159E)  produces viruses with decreases in heparin-Sepharose binding and increases  in viremia but different levels of binding to HS-expressing cells and  virulence phenotypes in newborn CD-1 mice (Byrnes, A.P., Griffin, D.E.,  2000.	transcription
54308	3	334883	5	NULL	NULL	0	NULL	R157H			is					statement 1					NULL		0	NULL	NULL	NULL	abs-batch0620-0649_virology_347_1_16380143_s_4	16380143	However, substitution of histidine  for arginine at E2-157 (R157H) or glutamate for lysine at E2-159 (K159E)  produces viruses with decreases in heparin-Sepharose binding and increases  in viremia but different levels of binding to HS-expressing cells and  virulence phenotypes in newborn CD-1 mice (Byrnes, A.P., Griffin, D.E.,  2000.	transcription
54309	4	334883	5	NULL	NULL	0	NULL	K159E			is					statement 2					NULL		0	NULL	NULL	NULL	abs-batch0620-0649_virology_347_1_16380143_s_4	16380143	However, substitution of histidine  for arginine at E2-157 (R157H) or glutamate for lysine at E2-159 (K159E)  produces viruses with decreases in heparin-Sepharose binding and increases  in viremia but different levels of binding to HS-expressing cells and  virulence phenotypes in newborn CD-1 mice (Byrnes, A.P., Griffin, D.E.,  2000.	transcription
54310	5	334883	5	NULL	NULL	0	NULL	statement 3			increases					viremia					NULL	newborn CD-1 mice	0	NULL	NULL	NULL	abs-batch0620-0649_virology_347_1_16380143_s_4	16380143	However, substitution of histidine  for arginine at E2-157 (R157H) or glutamate for lysine at E2-159 (K159E)  produces viruses with decreases in heparin-Sepharose binding and increases  in viremia but different levels of binding to HS-expressing cells and  virulence phenotypes in newborn CD-1 mice (Byrnes, A.P., Griffin, D.E.,  2000.	transcription
54311	6	334883	5	NULL	NULL	0	NULL	statement 4			increases					viremia 					NULL	newborn CD-1 mice	0	NULL	NULL	NULL	abs-batch0620-0649_virology_347_1_16380143_s_4	16380143	However, substitution of histidine  for arginine at E2-157 (R157H) or glutamate for lysine at E2-159 (K159E)  produces viruses with decreases in heparin-Sepharose binding and increases  in viremia but different levels of binding to HS-expressing cells and  virulence phenotypes in newborn CD-1 mice (Byrnes, A.P., Griffin, D.E.,  2000.	transcription
52815	1	334883	6	NULL	NULL	0	NULL	histidine	NULL		is substituted for	NULL				arginine	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_virology_347_1_16380143_s_4	16380143	However, substitution of histidine  for arginine at E2-157 (R157H) or glutamate for lysine at E2-159 (K159E)  produces viruses with decreases in heparin-Sepharose binding and increases  in viremia but different levels of binding to HS-expressing cells and  virulence phenotypes in newborn CD-1 mice (Byrnes, A.P., Griffin, D.E.,  2000.	transcription
52816	2	334883	6	NULL	NULL	0	NULL	glutamate	NULL		is substituted for	NULL				lysine	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_virology_347_1_16380143_s_4	16380143	However, substitution of histidine  for arginine at E2-157 (R157H) or glutamate for lysine at E2-159 (K159E)  produces viruses with decreases in heparin-Sepharose binding and increases  in viremia but different levels of binding to HS-expressing cells and  virulence phenotypes in newborn CD-1 mice (Byrnes, A.P., Griffin, D.E.,  2000.	transcription
52818	3	334883	6	NULL	NULL	0	NULL		NULL		is	NULL		R157H		statement 1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_virology_347_1_16380143_s_4	16380143	However, substitution of histidine  for arginine at E2-157 (R157H) or glutamate for lysine at E2-159 (K159E)  produces viruses with decreases in heparin-Sepharose binding and increases  in viremia but different levels of binding to HS-expressing cells and  virulence phenotypes in newborn CD-1 mice (Byrnes, A.P., Griffin, D.E.,  2000.	transcription
52820	4	334883	6	NULL	NULL	0	NULL		NULL		is	NULL		K159E		statement 2	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_virology_347_1_16380143_s_4	16380143	However, substitution of histidine  for arginine at E2-157 (R157H) or glutamate for lysine at E2-159 (K159E)  produces viruses with decreases in heparin-Sepharose binding and increases  in viremia but different levels of binding to HS-expressing cells and  virulence phenotypes in newborn CD-1 mice (Byrnes, A.P., Griffin, D.E.,  2000.	transcription
52821	5	334883	6	NULL	NULL	0	NULL	statement 3	NULL		increases	NULL				viremia	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_virology_347_1_16380143_s_4	16380143	However, substitution of histidine  for arginine at E2-157 (R157H) or glutamate for lysine at E2-159 (K159E)  produces viruses with decreases in heparin-Sepharose binding and increases  in viremia but different levels of binding to HS-expressing cells and  virulence phenotypes in newborn CD-1 mice (Byrnes, A.P., Griffin, D.E.,  2000.	transcription
52822	6	334883	6	NULL	NULL	0	NULL	statement 4	NULL		increases	NULL				viremia	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_virology_347_1_16380143_s_4	16380143	However, substitution of histidine  for arginine at E2-157 (R157H) or glutamate for lysine at E2-159 (K159E)  produces viruses with decreases in heparin-Sepharose binding and increases  in viremia but different levels of binding to HS-expressing cells and  virulence phenotypes in newborn CD-1 mice (Byrnes, A.P., Griffin, D.E.,  2000.	transcription
52492	1	334884	5	NULL	NULL	0	NULL	alanine	NULL		stimulates	NULL	efficiently			glutamine	NULL	uptake of			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_108	15581847	As clearly demonstrated by the data in   Table 2, alanine, serine, asparagine and threonine efficiently stimulated both the [3]glutamine uptake and efflux; cysteine and valine stimulated the efflux much more  than the uptake of [3]glutamine, i.e., they are preferentially translocated from outside to inside; methionine,  glycine, histidine, glutamate, arginine, creatine and MeAIB were poorly or not transported.	transcription
52493	2	334884	5	NULL	NULL	0	NULL	alanine	NULL		stimulates	NULL	efficiently			efflux	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_108	15581847	As clearly demonstrated by the data in   Table 2, alanine, serine, asparagine and threonine efficiently stimulated both the [3]glutamine uptake and efflux; cysteine and valine stimulated the efflux much more  than the uptake of [3]glutamine, i.e., they are preferentially translocated from outside to inside; methionine,  glycine, histidine, glutamate, arginine, creatine and MeAIB were poorly or not transported.	transcription
52494	3	334884	5	NULL	NULL	0	NULL	serine	NULL		stimulates	NULL	efficiently			glutamine	NULL	uptake of			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_108	15581847	As clearly demonstrated by the data in   Table 2, alanine, serine, asparagine and threonine efficiently stimulated both the [3]glutamine uptake and efflux; cysteine and valine stimulated the efflux much more  than the uptake of [3]glutamine, i.e., they are preferentially translocated from outside to inside; methionine,  glycine, histidine, glutamate, arginine, creatine and MeAIB were poorly or not transported.	transcription
52495	4	334884	5	NULL	NULL	0	NULL	serine	NULL		stimulates	NULL	efficiently			efflux	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_108	15581847	As clearly demonstrated by the data in   Table 2, alanine, serine, asparagine and threonine efficiently stimulated both the [3]glutamine uptake and efflux; cysteine and valine stimulated the efflux much more  than the uptake of [3]glutamine, i.e., they are preferentially translocated from outside to inside; methionine,  glycine, histidine, glutamate, arginine, creatine and MeAIB were poorly or not transported.	transcription
52496	5	334884	5	NULL	NULL	0	NULL	asparagine	NULL		stimulates	NULL	efficiently			glutamine	NULL	uptake of			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_108	15581847	As clearly demonstrated by the data in   Table 2, alanine, serine, asparagine and threonine efficiently stimulated both the [3]glutamine uptake and efflux; cysteine and valine stimulated the efflux much more  than the uptake of [3]glutamine, i.e., they are preferentially translocated from outside to inside; methionine,  glycine, histidine, glutamate, arginine, creatine and MeAIB were poorly or not transported.	transcription
52497	6	334884	5	NULL	NULL	0	NULL	asparagine	NULL		stimulates	NULL	efficiently			efflux	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_108	15581847	As clearly demonstrated by the data in   Table 2, alanine, serine, asparagine and threonine efficiently stimulated both the [3]glutamine uptake and efflux; cysteine and valine stimulated the efflux much more  than the uptake of [3]glutamine, i.e., they are preferentially translocated from outside to inside; methionine,  glycine, histidine, glutamate, arginine, creatine and MeAIB were poorly or not transported.	transcription
52498	7	334884	5	NULL	NULL	0	NULL	threonine	NULL		stimulates	NULL	efficiently			glutamine	NULL	uptake of			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_108	15581847	As clearly demonstrated by the data in   Table 2, alanine, serine, asparagine and threonine efficiently stimulated both the [3]glutamine uptake and efflux; cysteine and valine stimulated the efflux much more  than the uptake of [3]glutamine, i.e., they are preferentially translocated from outside to inside; methionine,  glycine, histidine, glutamate, arginine, creatine and MeAIB were poorly or not transported.	transcription
52499	8	334884	5	NULL	NULL	0	NULL	threonine	NULL		stimulates	NULL	efficiently			efflux	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_108	15581847	As clearly demonstrated by the data in   Table 2, alanine, serine, asparagine and threonine efficiently stimulated both the [3]glutamine uptake and efflux; cysteine and valine stimulated the efflux much more  than the uptake of [3]glutamine, i.e., they are preferentially translocated from outside to inside; methionine,  glycine, histidine, glutamate, arginine, creatine and MeAIB were poorly or not transported.	transcription
52500	9	334884	5	NULL	NULL	0	NULL	cysteine	NULL		stimulates	NULL				efflux	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_108	15581847	As clearly demonstrated by the data in   Table 2, alanine, serine, asparagine and threonine efficiently stimulated both the [3]glutamine uptake and efflux; cysteine and valine stimulated the efflux much more  than the uptake of [3]glutamine, i.e., they are preferentially translocated from outside to inside; methionine,  glycine, histidine, glutamate, arginine, creatine and MeAIB were poorly or not transported.	transcription
52501	10	334884	5	NULL	NULL	0	NULL	cysteine	NULL		stimulates	NULL				glutamine	NULL	uptake of			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_108	15581847	As clearly demonstrated by the data in   Table 2, alanine, serine, asparagine and threonine efficiently stimulated both the [3]glutamine uptake and efflux; cysteine and valine stimulated the efflux much more  than the uptake of [3]glutamine, i.e., they are preferentially translocated from outside to inside; methionine,  glycine, histidine, glutamate, arginine, creatine and MeAIB were poorly or not transported.	transcription
52502	11	334884	5	NULL	NULL	0	NULL	statement 9	NULL		is more than	NULL				statement 10	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_108	15581847	As clearly demonstrated by the data in   Table 2, alanine, serine, asparagine and threonine efficiently stimulated both the [3]glutamine uptake and efflux; cysteine and valine stimulated the efflux much more  than the uptake of [3]glutamine, i.e., they are preferentially translocated from outside to inside; methionine,  glycine, histidine, glutamate, arginine, creatine and MeAIB were poorly or not transported.	transcription
52503	12	334884	5	NULL	NULL	0	NULL	valine	NULL		stimulates	NULL				efflux	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_108	15581847	As clearly demonstrated by the data in   Table 2, alanine, serine, asparagine and threonine efficiently stimulated both the [3]glutamine uptake and efflux; cysteine and valine stimulated the efflux much more  than the uptake of [3]glutamine, i.e., they are preferentially translocated from outside to inside; methionine,  glycine, histidine, glutamate, arginine, creatine and MeAIB were poorly or not transported.	transcription
52504	13	334884	5	NULL	NULL	0	NULL	valine	NULL		stimulates	NULL				glutamine	NULL	uptake of			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_108	15581847	As clearly demonstrated by the data in   Table 2, alanine, serine, asparagine and threonine efficiently stimulated both the [3]glutamine uptake and efflux; cysteine and valine stimulated the efflux much more  than the uptake of [3]glutamine, i.e., they are preferentially translocated from outside to inside; methionine,  glycine, histidine, glutamate, arginine, creatine and MeAIB were poorly or not transported.	transcription
52505	14	334884	5	NULL	NULL	0	NULL	statement 12	NULL		is more than	NULL				statement 13	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_108	15581847	As clearly demonstrated by the data in   Table 2, alanine, serine, asparagine and threonine efficiently stimulated both the [3]glutamine uptake and efflux; cysteine and valine stimulated the efflux much more  than the uptake of [3]glutamine, i.e., they are preferentially translocated from outside to inside; methionine,  glycine, histidine, glutamate, arginine, creatine and MeAIB were poorly or not transported.	transcription
52802	1	334884	6	NULL	NULL	0	NULL	alanine	NULL		stimulates	NULL	efficiently			glutamine	NULL	uptake of 			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_108	15581847	As clearly demonstrated by the data in   Table 2, alanine, serine, asparagine and threonine efficiently stimulated both the [3]glutamine uptake and efflux; cysteine and valine stimulated the efflux much more  than the uptake of [3]glutamine, i.e., they are preferentially translocated from outside to inside; methionine,  glycine, histidine, glutamate, arginine, creatine and MeAIB were poorly or not transported.	transcription
52803	2	334884	6	NULL	NULL	0	NULL	serine	NULL		stimulates	NULL	efficiently			glutamine	NULL	uptake of 			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_108	15581847	As clearly demonstrated by the data in   Table 2, alanine, serine, asparagine and threonine efficiently stimulated both the [3]glutamine uptake and efflux; cysteine and valine stimulated the efflux much more  than the uptake of [3]glutamine, i.e., they are preferentially translocated from outside to inside; methionine,  glycine, histidine, glutamate, arginine, creatine and MeAIB were poorly or not transported.	transcription
52804	3	334884	6	NULL	NULL	0	NULL	asparagine	NULL		stimulates	NULL	efficiently			glutamine	NULL	uptake of 			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_108	15581847	As clearly demonstrated by the data in   Table 2, alanine, serine, asparagine and threonine efficiently stimulated both the [3]glutamine uptake and efflux; cysteine and valine stimulated the efflux much more  than the uptake of [3]glutamine, i.e., they are preferentially translocated from outside to inside; methionine,  glycine, histidine, glutamate, arginine, creatine and MeAIB were poorly or not transported.	transcription
52823	4	334884	6	NULL	NULL	0	NULL	threonine	NULL		stimulates	NULL	efficiently			glutamine	NULL	uptake of 			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_108	15581847	As clearly demonstrated by the data in   Table 2, alanine, serine, asparagine and threonine efficiently stimulated both the [3]glutamine uptake and efflux; cysteine and valine stimulated the efflux much more  than the uptake of [3]glutamine, i.e., they are preferentially translocated from outside to inside; methionine,  glycine, histidine, glutamate, arginine, creatine and MeAIB were poorly or not transported.	transcription
52824	5	334884	6	NULL	NULL	0	NULL	alanine	NULL		stimulates	NULL	efficiently			glutamine efflux	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_108	15581847	As clearly demonstrated by the data in   Table 2, alanine, serine, asparagine and threonine efficiently stimulated both the [3]glutamine uptake and efflux; cysteine and valine stimulated the efflux much more  than the uptake of [3]glutamine, i.e., they are preferentially translocated from outside to inside; methionine,  glycine, histidine, glutamate, arginine, creatine and MeAIB were poorly or not transported.	transcription
52825	6	334884	6	NULL	NULL	0	NULL	serine	NULL		stimulates	NULL	efficiently			glutamine efflux	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_108	15581847	As clearly demonstrated by the data in   Table 2, alanine, serine, asparagine and threonine efficiently stimulated both the [3]glutamine uptake and efflux; cysteine and valine stimulated the efflux much more  than the uptake of [3]glutamine, i.e., they are preferentially translocated from outside to inside; methionine,  glycine, histidine, glutamate, arginine, creatine and MeAIB were poorly or not transported.	transcription
52827	7	334884	6	NULL	NULL	0	NULL	asparagine	NULL		stimulates	NULL	efficiently			glutamine efflux	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_108	15581847	As clearly demonstrated by the data in   Table 2, alanine, serine, asparagine and threonine efficiently stimulated both the [3]glutamine uptake and efflux; cysteine and valine stimulated the efflux much more  than the uptake of [3]glutamine, i.e., they are preferentially translocated from outside to inside; methionine,  glycine, histidine, glutamate, arginine, creatine and MeAIB were poorly or not transported.	transcription
52828	8	334884	6	NULL	NULL	0	NULL	cysteine	NULL		stimulates	NULL	preferentially			glutamine efflux	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_108	15581847	As clearly demonstrated by the data in   Table 2, alanine, serine, asparagine and threonine efficiently stimulated both the [3]glutamine uptake and efflux; cysteine and valine stimulated the efflux much more  than the uptake of [3]glutamine, i.e., they are preferentially translocated from outside to inside; methionine,  glycine, histidine, glutamate, arginine, creatine and MeAIB were poorly or not transported.	transcription
52829	9	334884	6	NULL	NULL	0	NULL	valine	NULL		stimulates	NULL	preferentially			glutamine efflux	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1667_2_122_s_108	15581847	As clearly demonstrated by the data in   Table 2, alanine, serine, asparagine and threonine efficiently stimulated both the [3]glutamine uptake and efflux; cysteine and valine stimulated the efflux much more  than the uptake of [3]glutamine, i.e., they are preferentially translocated from outside to inside; methionine,  glycine, histidine, glutamate, arginine, creatine and MeAIB were poorly or not transported.	transcription
52045	1	334885	5	NULL	NULL	0	NULL	Receptor 5.24	NULL		is activated by	NULL				L-amino acids	NULL	basic			NULL		NULL	NULL	NULL	NULL	gw60_neuron_23_3_487_s_80	10433261	Receptor 5.24 responds best to basic L-amino acids, showing roughly equivalent currents upon activation by arginine and lysine, smaller responses to neutral aliphatic L-amino acids (e.g., methionine, isoleucine, threonine, serine, alanine) and little or no response to acidic and aromatic L-amino acids (e.g., glutamate, aspartate, tyrosine, phenylalanine, tryptophan, histidine); the receptor is not activated by D-arginine (all amino acids referred to hereafter are L-isomers unless stated otherwise).	transcription
52046	2	334885	5	NULL	NULL	0	NULL	Receptor 5.24	NULL		is not activated by	NULL				D-arginine	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_23_3_487_s_80	10433261	Receptor 5.24 responds best to basic L-amino acids, showing roughly equivalent currents upon activation by arginine and lysine, smaller responses to neutral aliphatic L-amino acids (e.g., methionine, isoleucine, threonine, serine, alanine) and little or no response to acidic and aromatic L-amino acids (e.g., glutamate, aspartate, tyrosine, phenylalanine, tryptophan, histidine); the receptor is not activated by D-arginine (all amino acids referred to hereafter are L-isomers unless stated otherwise).	transcription
52047	3	334885	5	NULL	NULL	0	NULL	Receptor 5.24	NULL		is activated by	NULL				arginine	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_23_3_487_s_80	10433261	Receptor 5.24 responds best to basic L-amino acids, showing roughly equivalent currents upon activation by arginine and lysine, smaller responses to neutral aliphatic L-amino acids (e.g., methionine, isoleucine, threonine, serine, alanine) and little or no response to acidic and aromatic L-amino acids (e.g., glutamate, aspartate, tyrosine, phenylalanine, tryptophan, histidine); the receptor is not activated by D-arginine (all amino acids referred to hereafter are L-isomers unless stated otherwise).	transcription
52048	4	334885	5	NULL	NULL	0	NULL	Receptor 5.24	NULL		is activated by	NULL				lysine	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_23_3_487_s_80	10433261	Receptor 5.24 responds best to basic L-amino acids, showing roughly equivalent currents upon activation by arginine and lysine, smaller responses to neutral aliphatic L-amino acids (e.g., methionine, isoleucine, threonine, serine, alanine) and little or no response to acidic and aromatic L-amino acids (e.g., glutamate, aspartate, tyrosine, phenylalanine, tryptophan, histidine); the receptor is not activated by D-arginine (all amino acids referred to hereafter are L-isomers unless stated otherwise).	transcription
52049	5	334885	5	NULL	NULL	0	NULL	Receptor 5.24	NULL		is activated by	NULL	weakly			L-amino acids	NULL	neutral;;aliphatic			NULL		0	NULL	NULL	NULL	gw60_neuron_23_3_487_s_80	10433261	Receptor 5.24 responds best to basic L-amino acids, showing roughly equivalent currents upon activation by arginine and lysine, smaller responses to neutral aliphatic L-amino acids (e.g., methionine, isoleucine, threonine, serine, alanine) and little or no response to acidic and aromatic L-amino acids (e.g., glutamate, aspartate, tyrosine, phenylalanine, tryptophan, histidine); the receptor is not activated by D-arginine (all amino acids referred to hereafter are L-isomers unless stated otherwise).	transcription
52050	6	334885	5	NULL	NULL	0	NULL	methionine	NULL		is a type of	NULL				L-amino acid	NULL	neutral;;aliphatic			NULL		0	NULL	NULL	NULL	gw60_neuron_23_3_487_s_80	10433261	Receptor 5.24 responds best to basic L-amino acids, showing roughly equivalent currents upon activation by arginine and lysine, smaller responses to neutral aliphatic L-amino acids (e.g., methionine, isoleucine, threonine, serine, alanine) and little or no response to acidic and aromatic L-amino acids (e.g., glutamate, aspartate, tyrosine, phenylalanine, tryptophan, histidine); the receptor is not activated by D-arginine (all amino acids referred to hereafter are L-isomers unless stated otherwise).	transcription
52051	7	334885	5	NULL	NULL	0	NULL	isoleucine	NULL		is a type of	NULL				L-amino acid	NULL	neutral;;aliphatic			NULL		0	NULL	NULL	NULL	gw60_neuron_23_3_487_s_80	10433261	Receptor 5.24 responds best to basic L-amino acids, showing roughly equivalent currents upon activation by arginine and lysine, smaller responses to neutral aliphatic L-amino acids (e.g., methionine, isoleucine, threonine, serine, alanine) and little or no response to acidic and aromatic L-amino acids (e.g., glutamate, aspartate, tyrosine, phenylalanine, tryptophan, histidine); the receptor is not activated by D-arginine (all amino acids referred to hereafter are L-isomers unless stated otherwise).	transcription
52052	8	334885	5	NULL	NULL	0	NULL	threonine	NULL		is a type of	NULL				L-amino acid	NULL	neutral;;aliphatic			NULL		0	NULL	NULL	NULL	gw60_neuron_23_3_487_s_80	10433261	Receptor 5.24 responds best to basic L-amino acids, showing roughly equivalent currents upon activation by arginine and lysine, smaller responses to neutral aliphatic L-amino acids (e.g., methionine, isoleucine, threonine, serine, alanine) and little or no response to acidic and aromatic L-amino acids (e.g., glutamate, aspartate, tyrosine, phenylalanine, tryptophan, histidine); the receptor is not activated by D-arginine (all amino acids referred to hereafter are L-isomers unless stated otherwise).	transcription
52053	9	334885	5	NULL	NULL	0	NULL	serine	NULL		is a type of	NULL				L-amino acid	NULL	neutral;;aliphatic			NULL		0	NULL	NULL	NULL	gw60_neuron_23_3_487_s_80	10433261	Receptor 5.24 responds best to basic L-amino acids, showing roughly equivalent currents upon activation by arginine and lysine, smaller responses to neutral aliphatic L-amino acids (e.g., methionine, isoleucine, threonine, serine, alanine) and little or no response to acidic and aromatic L-amino acids (e.g., glutamate, aspartate, tyrosine, phenylalanine, tryptophan, histidine); the receptor is not activated by D-arginine (all amino acids referred to hereafter are L-isomers unless stated otherwise).	transcription
52054	10	334885	5	NULL	NULL	0	NULL	alanine	NULL		is a type of	NULL				L-amino acid	NULL	neutral;;aliphatic			NULL		0	NULL	NULL	NULL	gw60_neuron_23_3_487_s_80	10433261	Receptor 5.24 responds best to basic L-amino acids, showing roughly equivalent currents upon activation by arginine and lysine, smaller responses to neutral aliphatic L-amino acids (e.g., methionine, isoleucine, threonine, serine, alanine) and little or no response to acidic and aromatic L-amino acids (e.g., glutamate, aspartate, tyrosine, phenylalanine, tryptophan, histidine); the receptor is not activated by D-arginine (all amino acids referred to hereafter are L-isomers unless stated otherwise).	transcription
52055	11	334885	5	NULL	NULL	0	NULL	Receptor 5.24	NULL		is activated by	NULL	may			L-amino acids	NULL	acidic 			NULL		0	NULL	NULL	NULL	gw60_neuron_23_3_487_s_80	10433261	Receptor 5.24 responds best to basic L-amino acids, showing roughly equivalent currents upon activation by arginine and lysine, smaller responses to neutral aliphatic L-amino acids (e.g., methionine, isoleucine, threonine, serine, alanine) and little or no response to acidic and aromatic L-amino acids (e.g., glutamate, aspartate, tyrosine, phenylalanine, tryptophan, histidine); the receptor is not activated by D-arginine (all amino acids referred to hereafter are L-isomers unless stated otherwise).	transcription
52056	12	334885	5	NULL	NULL	0	NULL	glutamate	NULL		is a type of	NULL				L-amino acid	NULL	acidic			NULL		0	NULL	NULL	NULL	gw60_neuron_23_3_487_s_80	10433261	Receptor 5.24 responds best to basic L-amino acids, showing roughly equivalent currents upon activation by arginine and lysine, smaller responses to neutral aliphatic L-amino acids (e.g., methionine, isoleucine, threonine, serine, alanine) and little or no response to acidic and aromatic L-amino acids (e.g., glutamate, aspartate, tyrosine, phenylalanine, tryptophan, histidine); the receptor is not activated by D-arginine (all amino acids referred to hereafter are L-isomers unless stated otherwise).	transcription
52057	13	334885	5	NULL	NULL	0	NULL	aspartate	NULL		is a type of	NULL				L-amino acid	NULL	acidic			NULL		0	NULL	NULL	NULL	gw60_neuron_23_3_487_s_80	10433261	Receptor 5.24 responds best to basic L-amino acids, showing roughly equivalent currents upon activation by arginine and lysine, smaller responses to neutral aliphatic L-amino acids (e.g., methionine, isoleucine, threonine, serine, alanine) and little or no response to acidic and aromatic L-amino acids (e.g., glutamate, aspartate, tyrosine, phenylalanine, tryptophan, histidine); the receptor is not activated by D-arginine (all amino acids referred to hereafter are L-isomers unless stated otherwise).	transcription
52058	14	334885	5	NULL	NULL	0	NULL	Receptor 5.24	NULL		is activated by	NULL	may			L-amino acids	NULL	aromatic			NULL		0	NULL	NULL	NULL	gw60_neuron_23_3_487_s_80	10433261	Receptor 5.24 responds best to basic L-amino acids, showing roughly equivalent currents upon activation by arginine and lysine, smaller responses to neutral aliphatic L-amino acids (e.g., methionine, isoleucine, threonine, serine, alanine) and little or no response to acidic and aromatic L-amino acids (e.g., glutamate, aspartate, tyrosine, phenylalanine, tryptophan, histidine); the receptor is not activated by D-arginine (all amino acids referred to hereafter are L-isomers unless stated otherwise).	transcription
52059	15	334885	5	NULL	NULL	0	NULL	tyrosine	NULL		is a type of	NULL				L-amino acid	NULL	aromatic			NULL		0	NULL	NULL	NULL	gw60_neuron_23_3_487_s_80	10433261	Receptor 5.24 responds best to basic L-amino acids, showing roughly equivalent currents upon activation by arginine and lysine, smaller responses to neutral aliphatic L-amino acids (e.g., methionine, isoleucine, threonine, serine, alanine) and little or no response to acidic and aromatic L-amino acids (e.g., glutamate, aspartate, tyrosine, phenylalanine, tryptophan, histidine); the receptor is not activated by D-arginine (all amino acids referred to hereafter are L-isomers unless stated otherwise).	transcription
52060	16	334885	5	NULL	NULL	0	NULL	phenylalanine	NULL		is a type of	NULL				L-amino acid	NULL	aromatic			NULL		0	NULL	NULL	NULL	gw60_neuron_23_3_487_s_80	10433261	Receptor 5.24 responds best to basic L-amino acids, showing roughly equivalent currents upon activation by arginine and lysine, smaller responses to neutral aliphatic L-amino acids (e.g., methionine, isoleucine, threonine, serine, alanine) and little or no response to acidic and aromatic L-amino acids (e.g., glutamate, aspartate, tyrosine, phenylalanine, tryptophan, histidine); the receptor is not activated by D-arginine (all amino acids referred to hereafter are L-isomers unless stated otherwise).	transcription
52061	17	334885	5	NULL	NULL	0	NULL	tryptophan	NULL		is a type of	NULL				L-amino acid	NULL	aromatic			NULL		0	NULL	NULL	NULL	gw60_neuron_23_3_487_s_80	10433261	Receptor 5.24 responds best to basic L-amino acids, showing roughly equivalent currents upon activation by arginine and lysine, smaller responses to neutral aliphatic L-amino acids (e.g., methionine, isoleucine, threonine, serine, alanine) and little or no response to acidic and aromatic L-amino acids (e.g., glutamate, aspartate, tyrosine, phenylalanine, tryptophan, histidine); the receptor is not activated by D-arginine (all amino acids referred to hereafter are L-isomers unless stated otherwise).	transcription
52062	18	334885	5	NULL	NULL	0	NULL	histidine	NULL		is a type of	NULL				L-amino acid	NULL	aromatic			NULL		0	NULL	NULL	NULL	gw60_neuron_23_3_487_s_80	10433261	Receptor 5.24 responds best to basic L-amino acids, showing roughly equivalent currents upon activation by arginine and lysine, smaller responses to neutral aliphatic L-amino acids (e.g., methionine, isoleucine, threonine, serine, alanine) and little or no response to acidic and aromatic L-amino acids (e.g., glutamate, aspartate, tyrosine, phenylalanine, tryptophan, histidine); the receptor is not activated by D-arginine (all amino acids referred to hereafter are L-isomers unless stated otherwise).	transcription
52903	1	334885	6	NULL	NULL	0	NULL	Receptor 5.24	NULL		is not activated by	NULL				D-arginine	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_23_3_487_s_80	10433261	Receptor 5.24 responds best to basic L-amino acids, showing roughly equivalent currents upon activation by arginine and lysine, smaller responses to neutral aliphatic L-amino acids (e.g., methionine, isoleucine, threonine, serine, alanine) and little or no response to acidic and aromatic L-amino acids (e.g., glutamate, aspartate, tyrosine, phenylalanine, tryptophan, histidine); the receptor is not activated by D-arginine (all amino acids referred to hereafter are L-isomers unless stated otherwise).	transcription
52904	2	334885	6	NULL	NULL	0	NULL	arginine	NULL		activates	NULL				receptor 5.24	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_23_3_487_s_80	10433261	Receptor 5.24 responds best to basic L-amino acids, showing roughly equivalent currents upon activation by arginine and lysine, smaller responses to neutral aliphatic L-amino acids (e.g., methionine, isoleucine, threonine, serine, alanine) and little or no response to acidic and aromatic L-amino acids (e.g., glutamate, aspartate, tyrosine, phenylalanine, tryptophan, histidine); the receptor is not activated by D-arginine (all amino acids referred to hereafter are L-isomers unless stated otherwise).	transcription
52905	3	334885	6	NULL	NULL	0	NULL	lysine	NULL		activates	NULL				receptor 5.24	NULL				NULL		0	NULL	NULL	NULL	gw60_neuron_23_3_487_s_80	10433261	Receptor 5.24 responds best to basic L-amino acids, showing roughly equivalent currents upon activation by arginine and lysine, smaller responses to neutral aliphatic L-amino acids (e.g., methionine, isoleucine, threonine, serine, alanine) and little or no response to acidic and aromatic L-amino acids (e.g., glutamate, aspartate, tyrosine, phenylalanine, tryptophan, histidine); the receptor is not activated by D-arginine (all amino acids referred to hereafter are L-isomers unless stated otherwise).	transcription
52038	1	334886	5	NULL	NULL	0	NULL		NULL		contains	NULL			exon IIIb		NULL	dipeptide residues in		fl2 domain 	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_17_10222_s_123	7730326	Dipeptide Residues in the fl2 and E Domain of Alternate  Exon IIIb Indirectly Modify FGF-2 and FGF-7 Binding  The exon  IIIb sequence in both the FGFR1 and FGFR2 genes is distinguished from  exon IIIc and homologous sequences in the FGFR3 and FGFR4 genes by  histidine-serine (HS) residues at the NH terminus of the  fl2 domain combined with the absence of lysine-glutamate (KE) residues  within the E strand of Loop III ( Fig. 1).	transcription
52039	2	334886	5	NULL	NULL	0	NULL		NULL		contains	NULL			exon IIIb		NULL	dipeptide residues in		E Domain	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_17_10222_s_123	7730326	Dipeptide Residues in the fl2 and E Domain of Alternate  Exon IIIb Indirectly Modify FGF-2 and FGF-7 Binding  The exon  IIIb sequence in both the FGFR1 and FGFR2 genes is distinguished from  exon IIIc and homologous sequences in the FGFR3 and FGFR4 genes by  histidine-serine (HS) residues at the NH terminus of the  fl2 domain combined with the absence of lysine-glutamate (KE) residues  within the E strand of Loop III ( Fig. 1).	transcription
52040	3	334886	5	NULL	NULL	0	NULL	statement 1	NULL		modify	NULL	indirectly			FGF-2	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_17_10222_s_123	7730326	Dipeptide Residues in the fl2 and E Domain of Alternate  Exon IIIb Indirectly Modify FGF-2 and FGF-7 Binding  The exon  IIIb sequence in both the FGFR1 and FGFR2 genes is distinguished from  exon IIIc and homologous sequences in the FGFR3 and FGFR4 genes by  histidine-serine (HS) residues at the NH terminus of the  fl2 domain combined with the absence of lysine-glutamate (KE) residues  within the E strand of Loop III ( Fig. 1).	transcription
52041	4	334886	5	NULL	NULL	0	NULL	statement 1	NULL		modify	NULL	indirectly			FGF-2	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_17_10222_s_123	7730326	Dipeptide Residues in the fl2 and E Domain of Alternate  Exon IIIb Indirectly Modify FGF-2 and FGF-7 Binding  The exon  IIIb sequence in both the FGFR1 and FGFR2 genes is distinguished from  exon IIIc and homologous sequences in the FGFR3 and FGFR4 genes by  histidine-serine (HS) residues at the NH terminus of the  fl2 domain combined with the absence of lysine-glutamate (KE) residues  within the E strand of Loop III ( Fig. 1).	transcription
52042	5	334886	5	NULL	NULL	0	NULL	statement 1	NULL		modify	NULL	indirectly			FGF-7	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_17_10222_s_123	7730326	Dipeptide Residues in the fl2 and E Domain of Alternate  Exon IIIb Indirectly Modify FGF-2 and FGF-7 Binding  The exon  IIIb sequence in both the FGFR1 and FGFR2 genes is distinguished from  exon IIIc and homologous sequences in the FGFR3 and FGFR4 genes by  histidine-serine (HS) residues at the NH terminus of the  fl2 domain combined with the absence of lysine-glutamate (KE) residues  within the E strand of Loop III ( Fig. 1).	transcription
52043	6	334886	5	NULL	NULL	0	NULL	statement 2	NULL		modify	NULL	indirectly			FGF-7	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_17_10222_s_123	7730326	Dipeptide Residues in the fl2 and E Domain of Alternate  Exon IIIb Indirectly Modify FGF-2 and FGF-7 Binding  The exon  IIIb sequence in both the FGFR1 and FGFR2 genes is distinguished from  exon IIIc and homologous sequences in the FGFR3 and FGFR4 genes by  histidine-serine (HS) residues at the NH terminus of the  fl2 domain combined with the absence of lysine-glutamate (KE) residues  within the E strand of Loop III ( Fig. 1).	transcription
51887	1	334887	5	NULL	NULL	0	NULL	AChEs	NULL		interacts with	NULL		glutamate 347;;histidine 460			NULL		active site serine		NULL		0	NULL	NULL	NULL	gw60_insectbiochemmolbiol_28_8_581_s_121	9753768	Conservation of the primary structure to other AChEs was also indicated by the presence of key residues ( Fig. 2 and  Fig. 3) that are characteristic of cholinesterases ( B. microplus AChE amino acids are numbered from the start of the mature protein according to   Massoulie et al. (1992) and the corresponding amino acid residues for  T. californica are listed below in parentheses for reference): (i) the active site serine 222 (200) which is surrounded by the sequence FGESAG-this is present in all known cholinesterases; (ii) glutamate 347 (327) and histidine 460 (440) which interact with the active site serine to form the catalytic triad (  Sussman et al., 1991); and (iii) the choline binding site, tryptophan 103 (84).	transcription
51888	2	334887	5	NULL	NULL	0	NULL	statement 1	NULL		forms	NULL				catalytic triad	NULL				NULL		0	NULL	NULL	NULL	gw60_insectbiochemmolbiol_28_8_581_s_121	9753768	Conservation of the primary structure to other AChEs was also indicated by the presence of key residues ( Fig. 2 and  Fig. 3) that are characteristic of cholinesterases ( B. microplus AChE amino acids are numbered from the start of the mature protein according to   Massoulie et al. (1992) and the corresponding amino acid residues for  T. californica are listed below in parentheses for reference): (i) the active site serine 222 (200) which is surrounded by the sequence FGESAG-this is present in all known cholinesterases; (ii) glutamate 347 (327) and histidine 460 (440) which interact with the active site serine to form the catalytic triad (  Sussman et al., 1991); and (iii) the choline binding site, tryptophan 103 (84).	transcription
52901	1	334887	6	NULL	NULL	0	NULL		NULL		interacts with	NULL		histidine 460			NULL		active site serine		NULL		0	NULL	NULL	NULL	gw60_insectbiochemmolbiol_28_8_581_s_121	9753768	Conservation of the primary structure to other AChEs was also indicated by the presence of key residues ( Fig. 2 and  Fig. 3) that are characteristic of cholinesterases ( B. microplus AChE amino acids are numbered from the start of the mature protein according to   Massoulie et al. (1992) and the corresponding amino acid residues for  T. californica are listed below in parentheses for reference): (i) the active site serine 222 (200) which is surrounded by the sequence FGESAG-this is present in all known cholinesterases; (ii) glutamate 347 (327) and histidine 460 (440) which interact with the active site serine to form the catalytic triad (  Sussman et al., 1991); and (iii) the choline binding site, tryptophan 103 (84).	transcription
52902	2	334887	6	NULL	NULL	0	NULL	statement 1	NULL		forms 	NULL				catalytic triad	NULL				NULL		0	NULL	NULL	NULL	gw60_insectbiochemmolbiol_28_8_581_s_121	9753768	Conservation of the primary structure to other AChEs was also indicated by the presence of key residues ( Fig. 2 and  Fig. 3) that are characteristic of cholinesterases ( B. microplus AChE amino acids are numbered from the start of the mature protein according to   Massoulie et al. (1992) and the corresponding amino acid residues for  T. californica are listed below in parentheses for reference): (i) the active site serine 222 (200) which is surrounded by the sequence FGESAG-this is present in all known cholinesterases; (ii) glutamate 347 (327) and histidine 460 (440) which interact with the active site serine to form the catalytic triad (  Sussman et al., 1991); and (iii) the choline binding site, tryptophan 103 (84).	transcription
51885	1	334888	5	NULL	NULL	0	NULL	alpha-glucose-1-phosphate	NULL		is converted to	NULL				glucose-6-phosphate	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_73_10_6935_s_64	16177373	The specific activity of PGM in cell extracts was measured as the conversion of alpha-glucose-1-phosphate to glucose-6-phosphate in a reaction coupled to reduction of glucose-6-phosphate by glucose-6-phosphate dehydrogenase and quantitated spectrophotometrically at 340 nm by monitoring the formation of NADPH from NADP+ at 30 degrees C.	transcription
51886	2	334888	5	NULL	NULL	0	NULL	glucose-6-phosphate dehydrogenase	NULL		reduces	NULL				glucose-6-phosphate	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_73_10_6935_s_64	16177373	The specific activity of PGM in cell extracts was measured as the conversion of alpha-glucose-1-phosphate to glucose-6-phosphate in a reaction coupled to reduction of glucose-6-phosphate by glucose-6-phosphate dehydrogenase and quantitated spectrophotometrically at 340 nm by monitoring the formation of NADPH from NADP+ at 30 degrees C.	transcription
52899	1	334888	6	NULL	NULL	0	NULL	alpha-glucose-1-phosphate	NULL		is converted to	NULL				glucose-6-phosphate	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_73_10_6935_s_64	16177373	The specific activity of PGM in cell extracts was measured as the conversion of alpha-glucose-1-phosphate to glucose-6-phosphate in a reaction coupled to reduction of glucose-6-phosphate by glucose-6-phosphate dehydrogenase and quantitated spectrophotometrically at 340 nm by monitoring the formation of NADPH from NADP+ at 30 degrees C.	transcription
52900	2	334888	6	NULL	NULL	0	NULL	glucose-6-phosphate dehydrogenase	NULL		reduces	NULL				glucose-6-phosphate	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_73_10_6935_s_64	16177373	The specific activity of PGM in cell extracts was measured as the conversion of alpha-glucose-1-phosphate to glucose-6-phosphate in a reaction coupled to reduction of glucose-6-phosphate by glucose-6-phosphate dehydrogenase and quantitated spectrophotometrically at 340 nm by monitoring the formation of NADPH from NADP+ at 30 degrees C.	transcription
51868	1	334889	5	NULL	NULL	0	NULL	UDP-glucose	NULL		is synthesized from	NULL				glucose-1-phosphate & UTP	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_72_7_4224_s_191	15213167	While the  galU gene product is responsible for synthesis of UDP-glucose from glucose-1-phosphate and UTP, the  algC gene encodes a bifunctional enzyme with both a phosphoglucomutase activity, which interconverts glucose-6-phosphate and glucose-1-phosphate, and a phosphomannomutase activity ( ,  ).	transcription
51869	2	334889	5	NULL	NULL	0	NULL	galU gene product	NULL		is responsible for	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_72_7_4224_s_191	15213167	While the  galU gene product is responsible for synthesis of UDP-glucose from glucose-1-phosphate and UTP, the  algC gene encodes a bifunctional enzyme with both a phosphoglucomutase activity, which interconverts glucose-6-phosphate and glucose-1-phosphate, and a phosphomannomutase activity ( ,  ).	transcription
51870	3	334889	5	NULL	NULL	0	NULL	algC gene	NULL		encodes	NULL				bifunctional enzyme	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_72_7_4224_s_191	15213167	While the  galU gene product is responsible for synthesis of UDP-glucose from glucose-1-phosphate and UTP, the  algC gene encodes a bifunctional enzyme with both a phosphoglucomutase activity, which interconverts glucose-6-phosphate and glucose-1-phosphate, and a phosphomannomutase activity ( ,  ).	transcription
52063	4	334889	5	NULL	NULL	0	NULL	algC gene	NULL		contains	NULL				phosphoglucomutase activity	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_72_7_4224_s_191	15213167	While the  galU gene product is responsible for synthesis of UDP-glucose from glucose-1-phosphate and UTP, the  algC gene encodes a bifunctional enzyme with both a phosphoglucomutase activity, which interconverts glucose-6-phosphate and glucose-1-phosphate, and a phosphomannomutase activity ( ,  ).	transcription
52064	5	334889	5	NULL	NULL	0	NULL	algC gene	NULL		contains	NULL				phosphomannomutase activity	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_72_7_4224_s_191	15213167	While the  galU gene product is responsible for synthesis of UDP-glucose from glucose-1-phosphate and UTP, the  algC gene encodes a bifunctional enzyme with both a phosphoglucomutase activity, which interconverts glucose-6-phosphate and glucose-1-phosphate, and a phosphomannomutase activity ( ,  ).	transcription
52065	6	334889	5	NULL	NULL	0	NULL	glucose-6-phosphate	NULL		is converted to	NULL				glucose-1-phosphate	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_72_7_4224_s_191	15213167	While the  galU gene product is responsible for synthesis of UDP-glucose from glucose-1-phosphate and UTP, the  algC gene encodes a bifunctional enzyme with both a phosphoglucomutase activity, which interconverts glucose-6-phosphate and glucose-1-phosphate, and a phosphomannomutase activity ( ,  ).	transcription
52066	7	334889	5	NULL	NULL	0	NULL	glucose-1-phosphate	NULL		is converted to	NULL				glucose-6-phosphate	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_72_7_4224_s_191	15213167	While the  galU gene product is responsible for synthesis of UDP-glucose from glucose-1-phosphate and UTP, the  algC gene encodes a bifunctional enzyme with both a phosphoglucomutase activity, which interconverts glucose-6-phosphate and glucose-1-phosphate, and a phosphomannomutase activity ( ,  ).	transcription
52067	8	334889	5	NULL	NULL	0	NULL	statement 3	NULL		catalyzes	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_72_7_4224_s_191	15213167	While the  galU gene product is responsible for synthesis of UDP-glucose from glucose-1-phosphate and UTP, the  algC gene encodes a bifunctional enzyme with both a phosphoglucomutase activity, which interconverts glucose-6-phosphate and glucose-1-phosphate, and a phosphomannomutase activity ( ,  ).	transcription
52068	9	334889	5	NULL	NULL	0	NULL	statement 3	NULL		catalyzes	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_72_7_4224_s_191	15213167	While the  galU gene product is responsible for synthesis of UDP-glucose from glucose-1-phosphate and UTP, the  algC gene encodes a bifunctional enzyme with both a phosphoglucomutase activity, which interconverts glucose-6-phosphate and glucose-1-phosphate, and a phosphomannomutase activity ( ,  ).	transcription
52881	1	334889	6	NULL	NULL	0	NULL	UDP-glucose	NULL		is synthesized from	NULL				glucose-1-phosphate	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_72_7_4224_s_191	15213167	While the  galU gene product is responsible for synthesis of UDP-glucose from glucose-1-phosphate and UTP, the  algC gene encodes a bifunctional enzyme with both a phosphoglucomutase activity, which interconverts glucose-6-phosphate and glucose-1-phosphate, and a phosphomannomutase activity ( ,  ).	transcription
52882	2	334889	6	NULL	NULL	0	NULL	UDP-glucose	NULL		is synthesized from	NULL				UTP	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_72_7_4224_s_191	15213167	While the  galU gene product is responsible for synthesis of UDP-glucose from glucose-1-phosphate and UTP, the  algC gene encodes a bifunctional enzyme with both a phosphoglucomutase activity, which interconverts glucose-6-phosphate and glucose-1-phosphate, and a phosphomannomutase activity ( ,  ).	transcription
52883	3	334889	6	NULL	NULL	0	NULL	statement 1	NULL		occurs simultaneously with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_72_7_4224_s_191	15213167	While the  galU gene product is responsible for synthesis of UDP-glucose from glucose-1-phosphate and UTP, the  algC gene encodes a bifunctional enzyme with both a phosphoglucomutase activity, which interconverts glucose-6-phosphate and glucose-1-phosphate, and a phosphomannomutase activity ( ,  ).	transcription
52884	4	334889	6	NULL	NULL	0	NULL	galU gene product	NULL		is responsible for	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_72_7_4224_s_191	15213167	While the  galU gene product is responsible for synthesis of UDP-glucose from glucose-1-phosphate and UTP, the  algC gene encodes a bifunctional enzyme with both a phosphoglucomutase activity, which interconverts glucose-6-phosphate and glucose-1-phosphate, and a phosphomannomutase activity ( ,  ).	transcription
52885	5	334889	6	NULL	NULL	0	NULL	galU gene product	NULL		is responsible for	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_72_7_4224_s_191	15213167	While the  galU gene product is responsible for synthesis of UDP-glucose from glucose-1-phosphate and UTP, the  algC gene encodes a bifunctional enzyme with both a phosphoglucomutase activity, which interconverts glucose-6-phosphate and glucose-1-phosphate, and a phosphomannomutase activity ( ,  ).	transcription
52886	6	334889	6	NULL	NULL	0	NULL	algC gene product	NULL		encodes	NULL				bifunctional enzyme	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_72_7_4224_s_191	15213167	While the  galU gene product is responsible for synthesis of UDP-glucose from glucose-1-phosphate and UTP, the  algC gene encodes a bifunctional enzyme with both a phosphoglucomutase activity, which interconverts glucose-6-phosphate and glucose-1-phosphate, and a phosphomannomutase activity ( ,  ).	transcription
52887	7	334889	6	NULL	NULL	0	NULL	algC gene product	NULL		exhibits	NULL				phosphoglucomutase activity	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_72_7_4224_s_191	15213167	While the  galU gene product is responsible for synthesis of UDP-glucose from glucose-1-phosphate and UTP, the  algC gene encodes a bifunctional enzyme with both a phosphoglucomutase activity, which interconverts glucose-6-phosphate and glucose-1-phosphate, and a phosphomannomutase activity ( ,  ).	transcription
52888	8	334889	6	NULL	NULL	0	NULL	algC gene product	NULL		exhibits	NULL				phosphomannomutase activity	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_72_7_4224_s_191	15213167	While the  galU gene product is responsible for synthesis of UDP-glucose from glucose-1-phosphate and UTP, the  algC gene encodes a bifunctional enzyme with both a phosphoglucomutase activity, which interconverts glucose-6-phosphate and glucose-1-phosphate, and a phosphomannomutase activity ( ,  ).	transcription
52889	9	334889	6	NULL	NULL	0	NULL	glucose-6-phosphate	NULL		is interconverted to	NULL				glucose-1-phosphate	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_72_7_4224_s_191	15213167	While the  galU gene product is responsible for synthesis of UDP-glucose from glucose-1-phosphate and UTP, the  algC gene encodes a bifunctional enzyme with both a phosphoglucomutase activity, which interconverts glucose-6-phosphate and glucose-1-phosphate, and a phosphomannomutase activity ( ,  ).	transcription
52890	10	334889	6	NULL	NULL	0	NULL	algC gene product	NULL		plays a role in	NULL				statement 9	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_72_7_4224_s_191	15213167	While the  galU gene product is responsible for synthesis of UDP-glucose from glucose-1-phosphate and UTP, the  algC gene encodes a bifunctional enzyme with both a phosphoglucomutase activity, which interconverts glucose-6-phosphate and glucose-1-phosphate, and a phosphomannomutase activity ( ,  ).	transcription
51871	1	334890	5	NULL	NULL	0	NULL	glucose-6-phosphate	NULL		is converted to	NULL				glucose-1-phosphate	NULL				NULL		0	NULL	NULL	NULL	abs-batch0560-0569_j-bacteriol_183_11_11344144_s_6	11344144	Pgm catalyzes the conversion of glucose-6-phosphate  to glucose-1-phosphate during growth on glucose, and therefore loss of  Pgm results in a deficiency in a variety of cellular constituents derived  from glucose-1-phosphate, including trehalose.	transcription
51872	2	334890	5	NULL	NULL	0	NULL	Pgm	NULL		catalyzes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0560-0569_j-bacteriol_183_11_11344144_s_6	11344144	Pgm catalyzes the conversion of glucose-6-phosphate  to glucose-1-phosphate during growth on glucose, and therefore loss of  Pgm results in a deficiency in a variety of cellular constituents derived  from glucose-1-phosphate, including trehalose.	transcription
51873	3	334890	5	NULL	NULL	0	NULL	statement 1	NULL		occurs during	NULL				growth on glucose	NULL				NULL		0	NULL	NULL	NULL	abs-batch0560-0569_j-bacteriol_183_11_11344144_s_6	11344144	Pgm catalyzes the conversion of glucose-6-phosphate  to glucose-1-phosphate during growth on glucose, and therefore loss of  Pgm results in a deficiency in a variety of cellular constituents derived  from glucose-1-phosphate, including trehalose.	transcription
51874	4	334890	5	NULL	NULL	0	NULL	Pgm	NULL	loss of	results in	NULL				trehalose	NULL	deficiency in			NULL		0	NULL	NULL	NULL	abs-batch0560-0569_j-bacteriol_183_11_11344144_s_6	11344144	Pgm catalyzes the conversion of glucose-6-phosphate  to glucose-1-phosphate during growth on glucose, and therefore loss of  Pgm results in a deficiency in a variety of cellular constituents derived  from glucose-1-phosphate, including trehalose.	transcription
52879	1	334890	6	NULL	NULL	0	NULL	glucose-6-phosphate	NULL		is converted to	NULL				glucose-1-phosphate	NULL				NULL		0	NULL	NULL	NULL	abs-batch0560-0569_j-bacteriol_183_11_11344144_s_6	11344144	Pgm catalyzes the conversion of glucose-6-phosphate  to glucose-1-phosphate during growth on glucose, and therefore loss of  Pgm results in a deficiency in a variety of cellular constituents derived  from glucose-1-phosphate, including trehalose.	transcription
52880	2	334890	6	NULL	NULL	0	NULL	Pgm	NULL		catalyzes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0560-0569_j-bacteriol_183_11_11344144_s_6	11344144	Pgm catalyzes the conversion of glucose-6-phosphate  to glucose-1-phosphate during growth on glucose, and therefore loss of  Pgm results in a deficiency in a variety of cellular constituents derived  from glucose-1-phosphate, including trehalose.	transcription
51875	1	334891	5	NULL	NULL	0	NULL	GAPDH	NULL		is	NULL				glyceraldehyde-3-phosphate dehydrogenase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_5_3091_s_36	9006960	There is experimental evidence indicating that accelerated NADH production by glyceraldehyde-3-phosphate dehydrogenase (GAPDH), linked to an effective glycerol 3-phosphate shuttle transferring cytosolic reducing equivalents to the mitochondria ( 26,  27), mediates this action of glucose ( 25).	transcription
51876	2	334891	5	NULL	NULL	0	NULL	NADH	NULL		is produced by	NULL				GAPDH	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_5_3091_s_36	9006960	There is experimental evidence indicating that accelerated NADH production by glyceraldehyde-3-phosphate dehydrogenase (GAPDH), linked to an effective glycerol 3-phosphate shuttle transferring cytosolic reducing equivalents to the mitochondria ( 26,  27), mediates this action of glucose ( 25).	transcription
51877	3	334891	5	NULL	NULL	0	NULL	cytosolic reducing equivalents	NULL		is transfered to	NULL				mitochondria	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_5_3091_s_36	9006960	There is experimental evidence indicating that accelerated NADH production by glyceraldehyde-3-phosphate dehydrogenase (GAPDH), linked to an effective glycerol 3-phosphate shuttle transferring cytosolic reducing equivalents to the mitochondria ( 26,  27), mediates this action of glucose ( 25).	transcription
51878	4	334891	5	NULL	NULL	0	NULL	glycerol 3-phosphate shuttle	NULL		is required for	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_5_3091_s_36	9006960	There is experimental evidence indicating that accelerated NADH production by glyceraldehyde-3-phosphate dehydrogenase (GAPDH), linked to an effective glycerol 3-phosphate shuttle transferring cytosolic reducing equivalents to the mitochondria ( 26,  27), mediates this action of glucose ( 25).	transcription
51879	5	334891	5	NULL	NULL	0	NULL	statement 1	NULL	accelerated	is linked to	NULL				statement 4	NULL	effective			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_5_3091_s_36	9006960	There is experimental evidence indicating that accelerated NADH production by glyceraldehyde-3-phosphate dehydrogenase (GAPDH), linked to an effective glycerol 3-phosphate shuttle transferring cytosolic reducing equivalents to the mitochondria ( 26,  27), mediates this action of glucose ( 25).	transcription
52877	1	334891	6	NULL	NULL	0	NULL	GAPDH	NULL		accelerates 	NULL				NADH	NULL	production of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_5_3091_s_36	9006960	There is experimental evidence indicating that accelerated NADH production by glyceraldehyde-3-phosphate dehydrogenase (GAPDH), linked to an effective glycerol 3-phosphate shuttle transferring cytosolic reducing equivalents to the mitochondria ( 26,  27), mediates this action of glucose ( 25).	transcription
52878	2	334891	6	NULL	NULL	0	NULL	GAPDH	NULL		is	NULL				glyceraldehyde-3-phosphate dehydrogenase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_5_3091_s_36	9006960	There is experimental evidence indicating that accelerated NADH production by glyceraldehyde-3-phosphate dehydrogenase (GAPDH), linked to an effective glycerol 3-phosphate shuttle transferring cytosolic reducing equivalents to the mitochondria ( 26,  27), mediates this action of glucose ( 25).	transcription
51880	1	334893	5	NULL	NULL	0	NULL	PII	NULL		interacts with	NULL				His6-NAGK	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_53_55202_s_227	15502156	C, interaction of PII with His6-NAGK in the presence of 1 mM ATP and 1 mM 2-oxoglutarate at various MgCl2 concentrations (1, 5, 10, and 20 mM).	transcription
51881	2	334893	5	NULL	NULL	0	NULL	statement 1	NULL		in the presence of	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_53_55202_s_227	15502156	C, interaction of PII with His6-NAGK in the presence of 1 mM ATP and 1 mM 2-oxoglutarate at various MgCl2 concentrations (1, 5, 10, and 20 mM).	transcription
51882	3	334893	5	NULL	NULL	0	NULL	statement 1	NULL		in the presence of	NULL				2-oxoglutarate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_53_55202_s_227	15502156	C, interaction of PII with His6-NAGK in the presence of 1 mM ATP and 1 mM 2-oxoglutarate at various MgCl2 concentrations (1, 5, 10, and 20 mM).	transcription
52874	1	334893	6	NULL	NULL	0	NULL	PII	NULL		interacts with	NULL				NAGK	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_53_55202_s_227	15502156	C, interaction of PII with His6-NAGK in the presence of 1 mM ATP and 1 mM 2-oxoglutarate at various MgCl2 concentrations (1, 5, 10, and 20 mM).	transcription
52875	2	334893	6	NULL	NULL	0	NULL	statement 1	NULL		occurs in presence of	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_53_55202_s_227	15502156	C, interaction of PII with His6-NAGK in the presence of 1 mM ATP and 1 mM 2-oxoglutarate at various MgCl2 concentrations (1, 5, 10, and 20 mM).	transcription
52876	3	334893	6	NULL	NULL	0	NULL	statement 1	NULL		occurs in presence of	NULL				2-oxoglutarate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_53_55202_s_227	15502156	C, interaction of PII with His6-NAGK in the presence of 1 mM ATP and 1 mM 2-oxoglutarate at various MgCl2 concentrations (1, 5, 10, and 20 mM).	transcription
51883	1	334894	5	NULL	NULL	0	NULL	ATP	NULL		bind	NULL				PII	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_53_55202_s_255	15502156	In the presence of 5 mM CaCl2, ATP photolabeling to PII was not impaired by the presence of NAGK, and 2-oxoglutarate stimulated ATP binding to PII both in the presence or absence of NAGK.	transcription
51884	2	334894	5	NULL	NULL	0	NULL	2-oxoglutarate	NULL		stimulates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_53_55202_s_255	15502156	In the presence of 5 mM CaCl2, ATP photolabeling to PII was not impaired by the presence of NAGK, and 2-oxoglutarate stimulated ATP binding to PII both in the presence or absence of NAGK.	transcription
52870	1	334894	6	NULL	NULL	0	NULL	ATP	NULL		bind	NULL				PII	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_53_55202_s_255	15502156	In the presence of 5 mM CaCl2, ATP photolabeling to PII was not impaired by the presence of NAGK, and 2-oxoglutarate stimulated ATP binding to PII both in the presence or absence of NAGK.	transcription
52871	2	334894	6	NULL	NULL	0	NULL	2-oxoglutarate	NULL		stimulates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_53_55202_s_255	15502156	In the presence of 5 mM CaCl2, ATP photolabeling to PII was not impaired by the presence of NAGK, and 2-oxoglutarate stimulated ATP binding to PII both in the presence or absence of NAGK.	transcription
52872	3	334894	6	NULL	NULL	0	NULL	ATP	NULL		is photolabeled to	NULL				PII	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_53_55202_s_255	15502156	In the presence of 5 mM CaCl2, ATP photolabeling to PII was not impaired by the presence of NAGK, and 2-oxoglutarate stimulated ATP binding to PII both in the presence or absence of NAGK.	transcription
52873	4	334894	6	NULL	NULL	0	NULL	NAGK	NULL		is not impaired by	NULL				statement 3	NULL	presence of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_53_55202_s_255	15502156	In the presence of 5 mM CaCl2, ATP photolabeling to PII was not impaired by the presence of NAGK, and 2-oxoglutarate stimulated ATP binding to PII both in the presence or absence of NAGK.	transcription
51889	1	334896	5	NULL	NULL	0	NULL	acetoacetyl:acyl CoA-transferase	NULL		catalyze	NULL				butyryl-CoA formation	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_16_4823_s_199	11466286	However, the genome encodes acetoacetyl:acyl CoA-transferase that catalyzes butyryl-CoA formation in solventogenesis (CAP0163-0164) and might also utilize succinate for the synthesis of succinyl-CoA and 2-oxoacid:ferredoxin oxidoreductase (CAC2458-2459) that could catalyze 2-oxoglutarate formation from succinyl-CoA (Fig.  5).	transcription
51890	2	334896	5	NULL	NULL	0	NULL	statement 1	NULL		occurs during	NULL				solventogenesis	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_16_4823_s_199	11466286	However, the genome encodes acetoacetyl:acyl CoA-transferase that catalyzes butyryl-CoA formation in solventogenesis (CAP0163-0164) and might also utilize succinate for the synthesis of succinyl-CoA and 2-oxoacid:ferredoxin oxidoreductase (CAC2458-2459) that could catalyze 2-oxoglutarate formation from succinyl-CoA (Fig.  5).	transcription
51891	3	334896	5	NULL	NULL	0	NULL	acetoacetyl:acyl CoA-transferase	NULL		utilize	NULL	might			succinate	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_16_4823_s_199	11466286	However, the genome encodes acetoacetyl:acyl CoA-transferase that catalyzes butyryl-CoA formation in solventogenesis (CAP0163-0164) and might also utilize succinate for the synthesis of succinyl-CoA and 2-oxoacid:ferredoxin oxidoreductase (CAC2458-2459) that could catalyze 2-oxoglutarate formation from succinyl-CoA (Fig.  5).	transcription
51892	4	334896	5	NULL	NULL	0	NULL	statement 3	NULL		is required for	NULL				succinyl-CoA	NULL	synthesis of			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_16_4823_s_199	11466286	However, the genome encodes acetoacetyl:acyl CoA-transferase that catalyzes butyryl-CoA formation in solventogenesis (CAP0163-0164) and might also utilize succinate for the synthesis of succinyl-CoA and 2-oxoacid:ferredoxin oxidoreductase (CAC2458-2459) that could catalyze 2-oxoglutarate formation from succinyl-CoA (Fig.  5).	transcription
51893	5	334896	5	NULL	NULL	0	NULL	2-oxoglutarate	NULL		is formed from	NULL				succinyl-CoA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_16_4823_s_199	11466286	However, the genome encodes acetoacetyl:acyl CoA-transferase that catalyzes butyryl-CoA formation in solventogenesis (CAP0163-0164) and might also utilize succinate for the synthesis of succinyl-CoA and 2-oxoacid:ferredoxin oxidoreductase (CAC2458-2459) that could catalyze 2-oxoglutarate formation from succinyl-CoA (Fig.  5).	transcription
51894	6	334896	5	NULL	NULL	0	NULL	2-oxoacid:ferredoxin oxidoreductase	NULL		catalyze	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_16_4823_s_199	11466286	However, the genome encodes acetoacetyl:acyl CoA-transferase that catalyzes butyryl-CoA formation in solventogenesis (CAP0163-0164) and might also utilize succinate for the synthesis of succinyl-CoA and 2-oxoacid:ferredoxin oxidoreductase (CAC2458-2459) that could catalyze 2-oxoglutarate formation from succinyl-CoA (Fig.  5).	transcription
51895	7	334896	5	NULL	NULL	0	NULL	2-oxoacid:ferredoxin oxidoreductase	NULL		is	NULL				CAC2458-2459	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_16_4823_s_199	11466286	However, the genome encodes acetoacetyl:acyl CoA-transferase that catalyzes butyryl-CoA formation in solventogenesis (CAP0163-0164) and might also utilize succinate for the synthesis of succinyl-CoA and 2-oxoacid:ferredoxin oxidoreductase (CAC2458-2459) that could catalyze 2-oxoglutarate formation from succinyl-CoA (Fig.  5).	transcription
51896	8	334896	5	NULL	NULL	0	NULL	acetoacetyl:acyl CoA-transferase	NULL		is	NULL				CAP0163-0164	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_16_4823_s_199	11466286	However, the genome encodes acetoacetyl:acyl CoA-transferase that catalyzes butyryl-CoA formation in solventogenesis (CAP0163-0164) and might also utilize succinate for the synthesis of succinyl-CoA and 2-oxoacid:ferredoxin oxidoreductase (CAC2458-2459) that could catalyze 2-oxoglutarate formation from succinyl-CoA (Fig.  5).	transcription
52864	1	334896	6	NULL	NULL	0	NULL	acetoacetyl:acyl CoA-transferase	NULL		catalyzes	NULL				butyryl-CoA	NULL	formation of 			NULL	solventogenesis (CAP0163-0164)	0	NULL	NULL	NULL	gw60_jbacteriol_183_16_4823_s_199	11466286	However, the genome encodes acetoacetyl:acyl CoA-transferase that catalyzes butyryl-CoA formation in solventogenesis (CAP0163-0164) and might also utilize succinate for the synthesis of succinyl-CoA and 2-oxoacid:ferredoxin oxidoreductase (CAC2458-2459) that could catalyze 2-oxoglutarate formation from succinyl-CoA (Fig.  5).	transcription
52865	2	334896	6	NULL	NULL	0	NULL	succinyl-CoA	NULL		forms	NULL				2-oxoglutarate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_16_4823_s_199	11466286	However, the genome encodes acetoacetyl:acyl CoA-transferase that catalyzes butyryl-CoA formation in solventogenesis (CAP0163-0164) and might also utilize succinate for the synthesis of succinyl-CoA and 2-oxoacid:ferredoxin oxidoreductase (CAC2458-2459) that could catalyze 2-oxoglutarate formation from succinyl-CoA (Fig.  5).	transcription
52866	3	334896	6	NULL	NULL	0	NULL	2-oxoacid:ferredoxin oxidoreductase	NULL		catalyzes	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_16_4823_s_199	11466286	However, the genome encodes acetoacetyl:acyl CoA-transferase that catalyzes butyryl-CoA formation in solventogenesis (CAP0163-0164) and might also utilize succinate for the synthesis of succinyl-CoA and 2-oxoacid:ferredoxin oxidoreductase (CAC2458-2459) that could catalyze 2-oxoglutarate formation from succinyl-CoA (Fig.  5).	transcription
52867	4	334896	6	NULL	NULL	0	NULL	2-oxoacid:ferredoxin oxidoreductase	NULL		is	NULL				CAC2458-2459	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_16_4823_s_199	11466286	However, the genome encodes acetoacetyl:acyl CoA-transferase that catalyzes butyryl-CoA formation in solventogenesis (CAP0163-0164) and might also utilize succinate for the synthesis of succinyl-CoA and 2-oxoacid:ferredoxin oxidoreductase (CAC2458-2459) that could catalyze 2-oxoglutarate formation from succinyl-CoA (Fig.  5).	transcription
52868	5	334896	6	NULL	NULL	0	NULL	succinate	NULL		is used for	NULL				succinyl-CoA	NULL	synthesis of 			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_16_4823_s_199	11466286	However, the genome encodes acetoacetyl:acyl CoA-transferase that catalyzes butyryl-CoA formation in solventogenesis (CAP0163-0164) and might also utilize succinate for the synthesis of succinyl-CoA and 2-oxoacid:ferredoxin oxidoreductase (CAC2458-2459) that could catalyze 2-oxoglutarate formation from succinyl-CoA (Fig.  5).	transcription
52869	6	334896	6	NULL	NULL	0	NULL	acetoacetyl:acyl CoA-transferase	NULL		plays a role in	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_16_4823_s_199	11466286	However, the genome encodes acetoacetyl:acyl CoA-transferase that catalyzes butyryl-CoA formation in solventogenesis (CAP0163-0164) and might also utilize succinate for the synthesis of succinyl-CoA and 2-oxoacid:ferredoxin oxidoreductase (CAC2458-2459) that could catalyze 2-oxoglutarate formation from succinyl-CoA (Fig.  5).	transcription
51897	1	334897	5	NULL	NULL	0	NULL	DHQ	NULL	oxygenation of	leads to	NULL				quercetin	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_21387_s_21	16702218	A recent  in vitro study on ANS revealed that ANS is capable of catalyzing the oxygenation of 2 R,3 R- trans-dihydroquercetin (DHQ)  5 toward quercetin  6; this reaction is also catalyzed by flavonol synthase (FLS), another member of the 2-oxoglutaratedependent dioxygenase family ( ).	transcription
51898	2	334897	5	NULL	NULL	0	NULL	ANS	NULL		catalyze	NULL				statement 1	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21387_s_21	16702218	A recent  in vitro study on ANS revealed that ANS is capable of catalyzing the oxygenation of 2 R,3 R- trans-dihydroquercetin (DHQ)  5 toward quercetin  6; this reaction is also catalyzed by flavonol synthase (FLS), another member of the 2-oxoglutaratedependent dioxygenase family ( ).	transcription
51899	3	334897	5	NULL	NULL	0	NULL	DHQ	NULL		is	NULL				2 R,3 R- trans-dihydroquercetin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21387_s_21	16702218	A recent  in vitro study on ANS revealed that ANS is capable of catalyzing the oxygenation of 2 R,3 R- trans-dihydroquercetin (DHQ)  5 toward quercetin  6; this reaction is also catalyzed by flavonol synthase (FLS), another member of the 2-oxoglutaratedependent dioxygenase family ( ).	transcription
51900	4	334897	5	NULL	NULL	0	NULL	FLS	NULL		is	NULL				flavonol synthase	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21387_s_21	16702218	A recent  in vitro study on ANS revealed that ANS is capable of catalyzing the oxygenation of 2 R,3 R- trans-dihydroquercetin (DHQ)  5 toward quercetin  6; this reaction is also catalyzed by flavonol synthase (FLS), another member of the 2-oxoglutaratedependent dioxygenase family ( ).	transcription
51901	5	334897	5	NULL	NULL	0	NULL	FLS	NULL		is a member of	NULL				2-oxoglutaratedependent dioxygenase family	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21387_s_21	16702218	A recent  in vitro study on ANS revealed that ANS is capable of catalyzing the oxygenation of 2 R,3 R- trans-dihydroquercetin (DHQ)  5 toward quercetin  6; this reaction is also catalyzed by flavonol synthase (FLS), another member of the 2-oxoglutaratedependent dioxygenase family ( ).	transcription
51902	6	334897	5	NULL	NULL	0	NULL	FLS	NULL		catalyze	NULL				statement 1	NULL				NULL	in vitro	0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21387_s_21	16702218	A recent  in vitro study on ANS revealed that ANS is capable of catalyzing the oxygenation of 2 R,3 R- trans-dihydroquercetin (DHQ)  5 toward quercetin  6; this reaction is also catalyzed by flavonol synthase (FLS), another member of the 2-oxoglutaratedependent dioxygenase family ( ).	transcription
52858	1	334897	6	NULL	NULL	0	NULL	DHQ 5	NULL		is catalyzed towards	NULL				quercetin 6	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21387_s_21	16702218	A recent  in vitro study on ANS revealed that ANS is capable of catalyzing the oxygenation of 2 R,3 R- trans-dihydroquercetin (DHQ)  5 toward quercetin  6; this reaction is also catalyzed by flavonol synthase (FLS), another member of the 2-oxoglutaratedependent dioxygenase family ( ).	transcription
52859	2	334897	6	NULL	NULL	0	NULL	DHQ	NULL		is 	NULL				2 R,3 R- trans-dihydroquercetin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21387_s_21	16702218	A recent  in vitro study on ANS revealed that ANS is capable of catalyzing the oxygenation of 2 R,3 R- trans-dihydroquercetin (DHQ)  5 toward quercetin  6; this reaction is also catalyzed by flavonol synthase (FLS), another member of the 2-oxoglutaratedependent dioxygenase family ( ).	transcription
52860	3	334897	6	NULL	NULL	0	NULL	ANS	NULL		catalyzes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21387_s_21	16702218	A recent  in vitro study on ANS revealed that ANS is capable of catalyzing the oxygenation of 2 R,3 R- trans-dihydroquercetin (DHQ)  5 toward quercetin  6; this reaction is also catalyzed by flavonol synthase (FLS), another member of the 2-oxoglutaratedependent dioxygenase family ( ).	transcription
52861	4	334897	6	NULL	NULL	0	NULL	FLS	NULL		catalyzes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21387_s_21	16702218	A recent  in vitro study on ANS revealed that ANS is capable of catalyzing the oxygenation of 2 R,3 R- trans-dihydroquercetin (DHQ)  5 toward quercetin  6; this reaction is also catalyzed by flavonol synthase (FLS), another member of the 2-oxoglutaratedependent dioxygenase family ( ).	transcription
52862	5	334897	6	NULL	NULL	0	NULL	FLS	NULL		is	NULL				flavonol synthase	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21387_s_21	16702218	A recent  in vitro study on ANS revealed that ANS is capable of catalyzing the oxygenation of 2 R,3 R- trans-dihydroquercetin (DHQ)  5 toward quercetin  6; this reaction is also catalyzed by flavonol synthase (FLS), another member of the 2-oxoglutaratedependent dioxygenase family ( ).	transcription
52863	6	334897	6	NULL	NULL	0	NULL	FLS	NULL		is a member of 	NULL				2-oxoglutaratedependent dioxygenase family	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21387_s_21	16702218	A recent  in vitro study on ANS revealed that ANS is capable of catalyzing the oxygenation of 2 R,3 R- trans-dihydroquercetin (DHQ)  5 toward quercetin  6; this reaction is also catalyzed by flavonol synthase (FLS), another member of the 2-oxoglutaratedependent dioxygenase family ( ).	transcription
51903	1	334898	5	NULL	NULL	0	NULL	NAD+ 	NULL		oxidizes	NULL				sorbitol	NULL				NULL		0	NULL	NULL	NULL	gw60_nature_414_6865_813_s_57	11742414	More recently, it has been proposed that oxidation of sorbitol by NAD+ increases the cytosolic NADH:NAD+ ratio, thereby inhibiting activity of the enzyme glyceraldehyde-3-phosphate dehydrogenase (GAPDH), and increasing concentrations of triose phosphate 14.	transcription
51904	2	334898	5	NULL	NULL	0	NULL	statement 1	NULL		increases	NULL				NADH:NAD+ ratio	NULL	cytosolic			NULL		0	NULL	NULL	NULL	gw60_nature_414_6865_813_s_57	11742414	More recently, it has been proposed that oxidation of sorbitol by NAD+ increases the cytosolic NADH:NAD+ ratio, thereby inhibiting activity of the enzyme glyceraldehyde-3-phosphate dehydrogenase (GAPDH), and increasing concentrations of triose phosphate 14.	transcription
51905	3	334898	5	NULL	NULL	0	NULL	statement 2	NULL		inhibit	NULL				GAPDH	NULL	activity of			NULL		0	NULL	NULL	NULL	gw60_nature_414_6865_813_s_57	11742414	More recently, it has been proposed that oxidation of sorbitol by NAD+ increases the cytosolic NADH:NAD+ ratio, thereby inhibiting activity of the enzyme glyceraldehyde-3-phosphate dehydrogenase (GAPDH), and increasing concentrations of triose phosphate 14.	transcription
51906	4	334898	5	NULL	NULL	0	NULL	GAPDH	NULL		is	NULL				glyceraldehyde-3-phosphate dehydrogenase	NULL				NULL		0	NULL	NULL	NULL	gw60_nature_414_6865_813_s_57	11742414	More recently, it has been proposed that oxidation of sorbitol by NAD+ increases the cytosolic NADH:NAD+ ratio, thereby inhibiting activity of the enzyme glyceraldehyde-3-phosphate dehydrogenase (GAPDH), and increasing concentrations of triose phosphate 14.	transcription
51907	5	334898	5	NULL	NULL	0	NULL	statement 2	NULL		increases	NULL				triose phosphate	NULL	concentration of			NULL		0	NULL	NULL	NULL	gw60_nature_414_6865_813_s_57	11742414	More recently, it has been proposed that oxidation of sorbitol by NAD+ increases the cytosolic NADH:NAD+ ratio, thereby inhibiting activity of the enzyme glyceraldehyde-3-phosphate dehydrogenase (GAPDH), and increasing concentrations of triose phosphate 14.	transcription
52853	1	334898	6	NULL	NULL	0	NULL	NAD+	NULL		oxidizes	NULL				sorbitol	NULL				NULL		0	NULL	NULL	NULL	gw60_nature_414_6865_813_s_57	11742414	More recently, it has been proposed that oxidation of sorbitol by NAD+ increases the cytosolic NADH:NAD+ ratio, thereby inhibiting activity of the enzyme glyceraldehyde-3-phosphate dehydrogenase (GAPDH), and increasing concentrations of triose phosphate 14.	transcription
52854	2	334898	6	NULL	NULL	0	NULL	statement 1	NULL		increases	NULL				NADH:NAD+ ratio	NULL	cytosolic			NULL		0	NULL	NULL	NULL	gw60_nature_414_6865_813_s_57	11742414	More recently, it has been proposed that oxidation of sorbitol by NAD+ increases the cytosolic NADH:NAD+ ratio, thereby inhibiting activity of the enzyme glyceraldehyde-3-phosphate dehydrogenase (GAPDH), and increasing concentrations of triose phosphate 14.	transcription
52855	3	334898	6	NULL	NULL	0	NULL	statement 2	NULL		inhibits	NULL				GAPDH	NULL	activity of 			NULL		0	NULL	NULL	NULL	gw60_nature_414_6865_813_s_57	11742414	More recently, it has been proposed that oxidation of sorbitol by NAD+ increases the cytosolic NADH:NAD+ ratio, thereby inhibiting activity of the enzyme glyceraldehyde-3-phosphate dehydrogenase (GAPDH), and increasing concentrations of triose phosphate 14.	transcription
52856	4	334898	6	NULL	NULL	0	NULL	GAPDH	NULL		is	NULL				glyceraldehyde-3-phosphate dehydrogenase	NULL				NULL		0	NULL	NULL	NULL	gw60_nature_414_6865_813_s_57	11742414	More recently, it has been proposed that oxidation of sorbitol by NAD+ increases the cytosolic NADH:NAD+ ratio, thereby inhibiting activity of the enzyme glyceraldehyde-3-phosphate dehydrogenase (GAPDH), and increasing concentrations of triose phosphate 14.	transcription
52857	5	334898	6	NULL	NULL	0	NULL	statement 2	NULL		increases	NULL				triose phosphate 14	NULL	concentrations of 			NULL		0	NULL	NULL	NULL	gw60_nature_414_6865_813_s_57	11742414	More recently, it has been proposed that oxidation of sorbitol by NAD+ increases the cytosolic NADH:NAD+ ratio, thereby inhibiting activity of the enzyme glyceraldehyde-3-phosphate dehydrogenase (GAPDH), and increasing concentrations of triose phosphate 14.	transcription
51908	1	334899	5	NULL	NULL	0	NULL	LCAT	NULL		is	NULL				lecithin:cholesterol acyltransferase	NULL				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_j-biomol-struct-dyn_24_1_16780378_s_2	16780378	Fluorescence spectroscopy has been used to investigate the conformational  changes that occur upon binding of wild type (WT) and mutant (Thr123Ile)  lecithin:cholesterol acyltransferase (LCAT) to the potential substrates  (dioleoyl-phosphatidyl choline [DOPC] and high density lipoprotein [HDL]).	transcription
51909	2	334899	5	NULL	NULL	0	NULL	DOPC	NULL		is	NULL				dioleoyl-phosphatidyl choline	NULL				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_j-biomol-struct-dyn_24_1_16780378_s_2	16780378	Fluorescence spectroscopy has been used to investigate the conformational  changes that occur upon binding of wild type (WT) and mutant (Thr123Ile)  lecithin:cholesterol acyltransferase (LCAT) to the potential substrates  (dioleoyl-phosphatidyl choline [DOPC] and high density lipoprotein [HDL]).	transcription
51910	3	334899	5	NULL	NULL	0	NULL	HDL	NULL		is	NULL				high density lipoprotein	NULL				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_j-biomol-struct-dyn_24_1_16780378_s_2	16780378	Fluorescence spectroscopy has been used to investigate the conformational  changes that occur upon binding of wild type (WT) and mutant (Thr123Ile)  lecithin:cholesterol acyltransferase (LCAT) to the potential substrates  (dioleoyl-phosphatidyl choline [DOPC] and high density lipoprotein [HDL]).	transcription
51911	4	334899	5	NULL	NULL	0	NULL	DOPC	NULL		is a substrate of	NULL	potential			LCAT	NULL				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_j-biomol-struct-dyn_24_1_16780378_s_2	16780378	Fluorescence spectroscopy has been used to investigate the conformational  changes that occur upon binding of wild type (WT) and mutant (Thr123Ile)  lecithin:cholesterol acyltransferase (LCAT) to the potential substrates  (dioleoyl-phosphatidyl choline [DOPC] and high density lipoprotein [HDL]).	transcription
51912	5	334899	5	NULL	NULL	0	NULL	HDL	NULL		is a substrate of	NULL	potential			LCAT	NULL				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_j-biomol-struct-dyn_24_1_16780378_s_2	16780378	Fluorescence spectroscopy has been used to investigate the conformational  changes that occur upon binding of wild type (WT) and mutant (Thr123Ile)  lecithin:cholesterol acyltransferase (LCAT) to the potential substrates  (dioleoyl-phosphatidyl choline [DOPC] and high density lipoprotein [HDL]).	transcription
52840	1	334899	6	NULL	NULL	0	NULL	LCAT	NULL	wild type	bind	NULL				DOPC	NULL				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_j-biomol-struct-dyn_24_1_16780378_s_2	16780378	Fluorescence spectroscopy has been used to investigate the conformational  changes that occur upon binding of wild type (WT) and mutant (Thr123Ile)  lecithin:cholesterol acyltransferase (LCAT) to the potential substrates  (dioleoyl-phosphatidyl choline [DOPC] and high density lipoprotein [HDL]).	transcription
52841	2	334899	6	NULL	NULL	0	NULL	LCAT	NULL		is	NULL				lecithin:cholesterol acyltransferase	NULL				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_j-biomol-struct-dyn_24_1_16780378_s_2	16780378	Fluorescence spectroscopy has been used to investigate the conformational  changes that occur upon binding of wild type (WT) and mutant (Thr123Ile)  lecithin:cholesterol acyltransferase (LCAT) to the potential substrates  (dioleoyl-phosphatidyl choline [DOPC] and high density lipoprotein [HDL]).	transcription
52842	3	334899	6	NULL	NULL	0	NULL	LCAT	NULL	mutant	bind	NULL		Thr123Ile		DOPC	NULL				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_j-biomol-struct-dyn_24_1_16780378_s_2	16780378	Fluorescence spectroscopy has been used to investigate the conformational  changes that occur upon binding of wild type (WT) and mutant (Thr123Ile)  lecithin:cholesterol acyltransferase (LCAT) to the potential substrates  (dioleoyl-phosphatidyl choline [DOPC] and high density lipoprotein [HDL]).	transcription
52849	4	334899	6	NULL	NULL	0	NULL	LCAT	NULL	wild type	bind	NULL				HDL	NULL				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_j-biomol-struct-dyn_24_1_16780378_s_2	16780378	Fluorescence spectroscopy has been used to investigate the conformational  changes that occur upon binding of wild type (WT) and mutant (Thr123Ile)  lecithin:cholesterol acyltransferase (LCAT) to the potential substrates  (dioleoyl-phosphatidyl choline [DOPC] and high density lipoprotein [HDL]).	transcription
52850	5	334899	6	NULL	NULL	0	NULL	LCAT	NULL	mutant	bind	NULL		Thr123Ile		HDL	NULL				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_j-biomol-struct-dyn_24_1_16780378_s_2	16780378	Fluorescence spectroscopy has been used to investigate the conformational  changes that occur upon binding of wild type (WT) and mutant (Thr123Ile)  lecithin:cholesterol acyltransferase (LCAT) to the potential substrates  (dioleoyl-phosphatidyl choline [DOPC] and high density lipoprotein [HDL]).	transcription
52851	6	334899	6	NULL	NULL	0	NULL	DOPC	NULL		is	NULL				dioleoyl-phosphatidyl choline	NULL				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_j-biomol-struct-dyn_24_1_16780378_s_2	16780378	Fluorescence spectroscopy has been used to investigate the conformational  changes that occur upon binding of wild type (WT) and mutant (Thr123Ile)  lecithin:cholesterol acyltransferase (LCAT) to the potential substrates  (dioleoyl-phosphatidyl choline [DOPC] and high density lipoprotein [HDL]).	transcription
52852	7	334899	6	NULL	NULL	0	NULL	HDL	NULL		is	NULL				high density lipoprotein	NULL				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_j-biomol-struct-dyn_24_1_16780378_s_2	16780378	Fluorescence spectroscopy has been used to investigate the conformational  changes that occur upon binding of wild type (WT) and mutant (Thr123Ile)  lecithin:cholesterol acyltransferase (LCAT) to the potential substrates  (dioleoyl-phosphatidyl choline [DOPC] and high density lipoprotein [HDL]).	transcription
51913	1	334900	5	NULL	NULL	0	NULL	PIP2	NULL		is	NULL				phosphatidylinositol 4, 5-biphosphate 	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_127_2_521_s_214	10385254	Stimulation of T cells through TCR results in the activation of PLCgammal which hydrolyzes the membrane phospholipid, phosphatidylinositol 4, 5-biphosphate (PIP2), into inositol 1, 4, 5-trisphosphate (IP3) and 1, 2-diacylglycerol (Isakov    et al.,  1987  ; Kikkawa & Nishizuka, 1986  ).	transcription
51914	2	334900	5	NULL	NULL	0	NULL	PIP2	NULL		is a type of	NULL				membrane phospholipid	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_127_2_521_s_214	10385254	Stimulation of T cells through TCR results in the activation of PLCgammal which hydrolyzes the membrane phospholipid, phosphatidylinositol 4, 5-biphosphate (PIP2), into inositol 1, 4, 5-trisphosphate (IP3) and 1, 2-diacylglycerol (Isakov    et al.,  1987  ; Kikkawa & Nishizuka, 1986  ).	transcription
51915	3	334900	5	NULL	NULL	0	NULL	IP3	NULL		is	NULL				inositol 1, 4, 5-trisphosphate	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_127_2_521_s_214	10385254	Stimulation of T cells through TCR results in the activation of PLCgammal which hydrolyzes the membrane phospholipid, phosphatidylinositol 4, 5-biphosphate (PIP2), into inositol 1, 4, 5-trisphosphate (IP3) and 1, 2-diacylglycerol (Isakov    et al.,  1987  ; Kikkawa & Nishizuka, 1986  ).	transcription
51916	4	334900	5	NULL	NULL	0	NULL	PIP2	NULL		is hydrolyzed to	NULL				IP3	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_127_2_521_s_214	10385254	Stimulation of T cells through TCR results in the activation of PLCgammal which hydrolyzes the membrane phospholipid, phosphatidylinositol 4, 5-biphosphate (PIP2), into inositol 1, 4, 5-trisphosphate (IP3) and 1, 2-diacylglycerol (Isakov    et al.,  1987  ; Kikkawa & Nishizuka, 1986  ).	transcription
51917	5	334900	5	NULL	NULL	0	NULL	PIP2	NULL		is hydrolyzed to	NULL				1, 2-diacylglycerol 	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_127_2_521_s_214	10385254	Stimulation of T cells through TCR results in the activation of PLCgammal which hydrolyzes the membrane phospholipid, phosphatidylinositol 4, 5-biphosphate (PIP2), into inositol 1, 4, 5-trisphosphate (IP3) and 1, 2-diacylglycerol (Isakov    et al.,  1987  ; Kikkawa & Nishizuka, 1986  ).	transcription
51918	6	334900	5	NULL	NULL	0	NULL	statement 4	NULL		occurs along with	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_127_2_521_s_214	10385254	Stimulation of T cells through TCR results in the activation of PLCgammal which hydrolyzes the membrane phospholipid, phosphatidylinositol 4, 5-biphosphate (PIP2), into inositol 1, 4, 5-trisphosphate (IP3) and 1, 2-diacylglycerol (Isakov    et al.,  1987  ; Kikkawa & Nishizuka, 1986  ).	transcription
51919	7	334900	5	NULL	NULL	0	NULL	PLCgammal	NULL	activated	catalyze	NULL				statement 6	NULL				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_127_2_521_s_214	10385254	Stimulation of T cells through TCR results in the activation of PLCgammal which hydrolyzes the membrane phospholipid, phosphatidylinositol 4, 5-biphosphate (PIP2), into inositol 1, 4, 5-trisphosphate (IP3) and 1, 2-diacylglycerol (Isakov    et al.,  1987  ; Kikkawa & Nishizuka, 1986  ).	transcription
51920	8	334900	5	NULL	NULL	0	NULL	T cells	NULL		is stimulated through	NULL				TCR	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_127_2_521_s_214	10385254	Stimulation of T cells through TCR results in the activation of PLCgammal which hydrolyzes the membrane phospholipid, phosphatidylinositol 4, 5-biphosphate (PIP2), into inositol 1, 4, 5-trisphosphate (IP3) and 1, 2-diacylglycerol (Isakov    et al.,  1987  ; Kikkawa & Nishizuka, 1986  ).	transcription
51921	9	334900	5	NULL	NULL	0	NULL	statement 8	NULL		activates	NULL				PLCgammal	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_127_2_521_s_214	10385254	Stimulation of T cells through TCR results in the activation of PLCgammal which hydrolyzes the membrane phospholipid, phosphatidylinositol 4, 5-biphosphate (PIP2), into inositol 1, 4, 5-trisphosphate (IP3) and 1, 2-diacylglycerol (Isakov    et al.,  1987  ; Kikkawa & Nishizuka, 1986  ).	transcription
52830	1	334900	6	NULL	NULL	0	NULL	TCR	NULL		stimulates	NULL				T cells	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_127_2_521_s_214	10385254	Stimulation of T cells through TCR results in the activation of PLCgammal which hydrolyzes the membrane phospholipid, phosphatidylinositol 4, 5-biphosphate (PIP2), into inositol 1, 4, 5-trisphosphate (IP3) and 1, 2-diacylglycerol (Isakov    et al.,  1987  ; Kikkawa & Nishizuka, 1986  ).	transcription
52831	2	334900	6	NULL	NULL	0	NULL	statement 1	NULL		results in	NULL				PLCgamma1	NULL	activation of 			NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_127_2_521_s_214	10385254	Stimulation of T cells through TCR results in the activation of PLCgammal which hydrolyzes the membrane phospholipid, phosphatidylinositol 4, 5-biphosphate (PIP2), into inositol 1, 4, 5-trisphosphate (IP3) and 1, 2-diacylglycerol (Isakov    et al.,  1987  ; Kikkawa & Nishizuka, 1986  ).	transcription
52832	3	334900	6	NULL	NULL	0	NULL	statement 2	NULL		hydrolyzes	NULL				PIP2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_127_2_521_s_214	10385254	Stimulation of T cells through TCR results in the activation of PLCgammal which hydrolyzes the membrane phospholipid, phosphatidylinositol 4, 5-biphosphate (PIP2), into inositol 1, 4, 5-trisphosphate (IP3) and 1, 2-diacylglycerol (Isakov    et al.,  1987  ; Kikkawa & Nishizuka, 1986  ).	transcription
52833	4	334900	6	NULL	NULL	0	NULL	PIP2	NULL		is	NULL				phosphatidylinositol 4, 5-biphosphate	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_127_2_521_s_214	10385254	Stimulation of T cells through TCR results in the activation of PLCgammal which hydrolyzes the membrane phospholipid, phosphatidylinositol 4, 5-biphosphate (PIP2), into inositol 1, 4, 5-trisphosphate (IP3) and 1, 2-diacylglycerol (Isakov    et al.,  1987  ; Kikkawa & Nishizuka, 1986  ).	transcription
52834	5	334900	6	NULL	NULL	0	NULL	PIP2	NULL		is a type of	NULL				membrane phospholipid	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_127_2_521_s_214	10385254	Stimulation of T cells through TCR results in the activation of PLCgammal which hydrolyzes the membrane phospholipid, phosphatidylinositol 4, 5-biphosphate (PIP2), into inositol 1, 4, 5-trisphosphate (IP3) and 1, 2-diacylglycerol (Isakov    et al.,  1987  ; Kikkawa & Nishizuka, 1986  ).	transcription
52835	6	334900	6	NULL	NULL	0	NULL	PIP2	NULL		is hydrolyzed into	NULL				IP3	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_127_2_521_s_214	10385254	Stimulation of T cells through TCR results in the activation of PLCgammal which hydrolyzes the membrane phospholipid, phosphatidylinositol 4, 5-biphosphate (PIP2), into inositol 1, 4, 5-trisphosphate (IP3) and 1, 2-diacylglycerol (Isakov    et al.,  1987  ; Kikkawa & Nishizuka, 1986  ).	transcription
52836	7	334900	6	NULL	NULL	0	NULL	PIP2	NULL		is hydrolyzed into	NULL				1, 2-diacylglycerol	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_127_2_521_s_214	10385254	Stimulation of T cells through TCR results in the activation of PLCgammal which hydrolyzes the membrane phospholipid, phosphatidylinositol 4, 5-biphosphate (PIP2), into inositol 1, 4, 5-trisphosphate (IP3) and 1, 2-diacylglycerol (Isakov    et al.,  1987  ; Kikkawa & Nishizuka, 1986  ).	transcription
52837	8	334900	6	NULL	NULL	0	NULL	IP3	NULL		is	NULL				inositol 1, 4, 5-trisphosphate	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_127_2_521_s_214	10385254	Stimulation of T cells through TCR results in the activation of PLCgammal which hydrolyzes the membrane phospholipid, phosphatidylinositol 4, 5-biphosphate (PIP2), into inositol 1, 4, 5-trisphosphate (IP3) and 1, 2-diacylglycerol (Isakov    et al.,  1987  ; Kikkawa & Nishizuka, 1986  ).	transcription
52838	9	334900	6	NULL	NULL	0	NULL	statement 3	NULL		leads to	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_127_2_521_s_214	10385254	Stimulation of T cells through TCR results in the activation of PLCgammal which hydrolyzes the membrane phospholipid, phosphatidylinositol 4, 5-biphosphate (PIP2), into inositol 1, 4, 5-trisphosphate (IP3) and 1, 2-diacylglycerol (Isakov    et al.,  1987  ; Kikkawa & Nishizuka, 1986  ).	transcription
52839	10	334900	6	NULL	NULL	0	NULL	statement 3	NULL		leads to	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_127_2_521_s_214	10385254	Stimulation of T cells through TCR results in the activation of PLCgammal which hydrolyzes the membrane phospholipid, phosphatidylinositol 4, 5-biphosphate (PIP2), into inositol 1, 4, 5-trisphosphate (IP3) and 1, 2-diacylglycerol (Isakov    et al.,  1987  ; Kikkawa & Nishizuka, 1986  ).	transcription
51922	1	334901	5	NULL	NULL	0	NULL	Pyruvate 	NULL		interacts with	NULL	directly			HPHs	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_180	16223732	Pyruvate and Oxaloacetate Directly Interact with HPHs --	transcription
51923	2	334901	5	NULL	NULL	0	NULL	Oxaloacetate	NULL		interacts with	NULL	directly			HPHs	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_180	16223732	Pyruvate and Oxaloacetate Directly Interact with HPHs --	transcription
53716	1	334901	6	NULL	NULL	0	NULL	Pyruvate			interacts with		directly			HPH					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_180	16223732	Pyruvate and Oxaloacetate Directly Interact with HPHs --	transcription
53717	2	334901	6	NULL	NULL	0	NULL	Oxaloacetate			interacts with		directly			HPH					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_180	16223732	Pyruvate and Oxaloacetate Directly Interact with HPHs --	transcription
51924	1	334902	5	NULL	NULL	0	NULL	pyruvate	NULL		is carboxylated to	NULL				oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw60_genomeres_12_11_1703_s_126	12421757	PYC2 catalyzes the carboxylation of pyruvate into oxaloacetate.	transcription
51925	2	334902	5	NULL	NULL	0	NULL	PYC2 	NULL		catalyze	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_genomeres_12_11_1703_s_126	12421757	PYC2 catalyzes the carboxylation of pyruvate into oxaloacetate.	transcription
53718	1	334902	6	NULL	NULL	0	NULL	pyruvate			is carboxylated to					oxaloacetate					NULL		0	NULL	NULL	NULL	gw60_genomeres_12_11_1703_s_126	12421757	PYC2 catalyzes the carboxylation of pyruvate into oxaloacetate.	transcription
53719	2	334902	6	NULL	NULL	0	NULL	PYC2			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw60_genomeres_12_11_1703_s_126	12421757	PYC2 catalyzes the carboxylation of pyruvate into oxaloacetate.	transcription
51926	1	334903	5	NULL	NULL	0	NULL	Pyruvate	NULL	carboxylation of	is catalyzed by	NULL				pyruvate carboxylase	NULL				NULL		0	NULL	NULL	NULL	gw60_diabetes_51_9_2669_s_11	12196457	Pyruvate carboxylation catalyzed by pyruvate carboxylase will supply oxaloacetate to mitochondrial aspartate aminotransferase.	transcription
51927	2	334903	5	NULL	NULL	0	NULL	oxaloacetate	NULL		is supplied to	NULL				aspartate aminotransferase	NULL	mitochondrial			NULL		0	NULL	NULL	NULL	gw60_diabetes_51_9_2669_s_11	12196457	Pyruvate carboxylation catalyzed by pyruvate carboxylase will supply oxaloacetate to mitochondrial aspartate aminotransferase.	transcription
51928	3	334903	5	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_diabetes_51_9_2669_s_11	12196457	Pyruvate carboxylation catalyzed by pyruvate carboxylase will supply oxaloacetate to mitochondrial aspartate aminotransferase.	transcription
53720	2	334903	6	NULL	NULL	0	NULL	pyruvate carboxylase			catalyzes					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_diabetes_51_9_2669_s_11	12196457	Pyruvate carboxylation catalyzed by pyruvate carboxylase will supply oxaloacetate to mitochondrial aspartate aminotransferase.	transcription
53721	1	334903	6	NULL	NULL	0	NULL	pyruvate			is carboxylated to					oxaloacetate					NULL		0	NULL	NULL	NULL	gw60_diabetes_51_9_2669_s_11	12196457	Pyruvate carboxylation catalyzed by pyruvate carboxylase will supply oxaloacetate to mitochondrial aspartate aminotransferase.	transcription
53722	3	334903	6	NULL	NULL	0	NULL	Oxaloacetate			is supplied to					aspartate aminotransferase		mitochondrial			NULL		0	NULL	NULL	NULL	gw60_diabetes_51_9_2669_s_11	12196457	Pyruvate carboxylation catalyzed by pyruvate carboxylase will supply oxaloacetate to mitochondrial aspartate aminotransferase.	transcription
53723	4	334903	6	NULL	NULL	0	NULL	statement 3			occurs due to					statement 1					NULL		0	NULL	NULL	NULL	gw60_diabetes_51_9_2669_s_11	12196457	Pyruvate carboxylation catalyzed by pyruvate carboxylase will supply oxaloacetate to mitochondrial aspartate aminotransferase.	transcription
51929	1	334904	5	NULL	NULL	0	NULL	pyruvate	NULL		is carboxylated to	NULL				oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_cell-mol-life-sci_63_7-8_16505973_s_2	16505973	Pyruvate carboxylase (PC) catalyzes the ATP-dependent carboxylation of  pyruvate to oxaloacetate.	transcription
51930	2	334904	5	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_cell-mol-life-sci_63_7-8_16505973_s_2	16505973	Pyruvate carboxylase (PC) catalyzes the ATP-dependent carboxylation of  pyruvate to oxaloacetate.	transcription
51931	3	334904	5	NULL	NULL	0	NULL	PC	NULL		catalyzes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_cell-mol-life-sci_63_7-8_16505973_s_2	16505973	Pyruvate carboxylase (PC) catalyzes the ATP-dependent carboxylation of  pyruvate to oxaloacetate.	transcription
51932	4	334904	5	NULL	NULL	0	NULL	PC	NULL		is	NULL				pyruvate carboxylase	NULL				NULL		0	NULL	NULL	NULL	abs-batch0680-0699_cell-mol-life-sci_63_7-8_16505973_s_2	16505973	Pyruvate carboxylase (PC) catalyzes the ATP-dependent carboxylation of  pyruvate to oxaloacetate.	transcription
53724	1	334904	6	NULL	NULL	0	NULL	PC			is					pyruvate carboxylase					NULL		0	NULL	NULL	NULL	abs-batch0680-0699_cell-mol-life-sci_63_7-8_16505973_s_2	16505973	Pyruvate carboxylase (PC) catalyzes the ATP-dependent carboxylation of  pyruvate to oxaloacetate.	transcription
53725	2	334904	6	NULL	NULL	0	NULL	pyruvate			is carboxylated to					oxaloacetate					NULL		0	NULL	NULL	NULL	abs-batch0680-0699_cell-mol-life-sci_63_7-8_16505973_s_2	16505973	Pyruvate carboxylase (PC) catalyzes the ATP-dependent carboxylation of  pyruvate to oxaloacetate.	transcription
53726	3	334904	6	NULL	NULL	0	NULL	PC			catalyzes					statement 2					NULL		0	NULL	NULL	NULL	abs-batch0680-0699_cell-mol-life-sci_63_7-8_16505973_s_2	16505973	Pyruvate carboxylase (PC) catalyzes the ATP-dependent carboxylation of  pyruvate to oxaloacetate.	transcription
53727	4	334904	6	NULL	NULL	0	NULL	statement 2			is dependent on					ATP					NULL		0	NULL	NULL	NULL	abs-batch0680-0699_cell-mol-life-sci_63_7-8_16505973_s_2	16505973	Pyruvate carboxylase (PC) catalyzes the ATP-dependent carboxylation of  pyruvate to oxaloacetate.	transcription
51933	1	334905	5	NULL	NULL	0	NULL	CHA	NULL		is converted to	NULL				pyruvate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_1_41_s_9	12486039	Electrospray-ionization mass spectrometry indicated that LigK catalyzes not only the conversion of CHA to pyruvate and oxaloacetate but also that of oxaloacetate to pyruvate and CO2.	transcription
51934	2	334905	5	NULL	NULL	0	NULL	CHA	NULL		is converted to	NULL				oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_1_41_s_9	12486039	Electrospray-ionization mass spectrometry indicated that LigK catalyzes not only the conversion of CHA to pyruvate and oxaloacetate but also that of oxaloacetate to pyruvate and CO2.	transcription
51935	3	334905	5	NULL	NULL	0	NULL	statement 1	NULL		occurs along with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_1_41_s_9	12486039	Electrospray-ionization mass spectrometry indicated that LigK catalyzes not only the conversion of CHA to pyruvate and oxaloacetate but also that of oxaloacetate to pyruvate and CO2.	transcription
51936	4	334905	5	NULL	NULL	0	NULL	LigK	NULL		catalyzes	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_1_41_s_9	12486039	Electrospray-ionization mass spectrometry indicated that LigK catalyzes not only the conversion of CHA to pyruvate and oxaloacetate but also that of oxaloacetate to pyruvate and CO2.	transcription
53728	1	334905	6	NULL	NULL	0	NULL	CHA			is converted to					pyruvate					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_1_41_s_9	12486039	Electrospray-ionization mass spectrometry indicated that LigK catalyzes not only the conversion of CHA to pyruvate and oxaloacetate but also that of oxaloacetate to pyruvate and CO2.	transcription
53729	2	334905	6	NULL	NULL	0	NULL	CHA			is converted to					oxaloacetate					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_1_41_s_9	12486039	Electrospray-ionization mass spectrometry indicated that LigK catalyzes not only the conversion of CHA to pyruvate and oxaloacetate but also that of oxaloacetate to pyruvate and CO2.	transcription
53730	3	334905	6	NULL	NULL	0	NULL	LigK			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_1_41_s_9	12486039	Electrospray-ionization mass spectrometry indicated that LigK catalyzes not only the conversion of CHA to pyruvate and oxaloacetate but also that of oxaloacetate to pyruvate and CO2.	transcription
53731	4	334905	6	NULL	NULL	0	NULL	LigK			catalyzes					statement 2					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_1_41_s_9	12486039	Electrospray-ionization mass spectrometry indicated that LigK catalyzes not only the conversion of CHA to pyruvate and oxaloacetate but also that of oxaloacetate to pyruvate and CO2.	transcription
53732	5	334905	6	NULL	NULL	0	NULL	Oxaloacetate			is catalyzed to					pyruvate					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_1_41_s_9	12486039	Electrospray-ionization mass spectrometry indicated that LigK catalyzes not only the conversion of CHA to pyruvate and oxaloacetate but also that of oxaloacetate to pyruvate and CO2.	transcription
53733	6	334905	6	NULL	NULL	0	NULL	Oxaloacetate			is catalyzed to					CO2					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_1_41_s_9	12486039	Electrospray-ionization mass spectrometry indicated that LigK catalyzes not only the conversion of CHA to pyruvate and oxaloacetate but also that of oxaloacetate to pyruvate and CO2.	transcription
53734	7	334905	6	NULL	NULL	0	NULL	LigK			catalyzes					statement 5					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_1_41_s_9	12486039	Electrospray-ionization mass spectrometry indicated that LigK catalyzes not only the conversion of CHA to pyruvate and oxaloacetate but also that of oxaloacetate to pyruvate and CO2.	transcription
53735	8	334905	6	NULL	NULL	0	NULL	LigK			catalyzes					statement 6					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_1_41_s_9	12486039	Electrospray-ionization mass spectrometry indicated that LigK catalyzes not only the conversion of CHA to pyruvate and oxaloacetate but also that of oxaloacetate to pyruvate and CO2.	transcription
52484	1	334906	5	NULL	NULL	0	NULL	citrate	NULL		is split into	NULL				oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_4_665_s_432	16339740	The conversion involves the splitting of citrate into oxaloacetate and acetate catalyzed by citrate lyase and the decarboxylation of oxaloacetate to pyruvate and carbon dioxide catalyzed by oxaloacetate decarboxylase.	transcription
52485	2	334906	5	NULL	NULL	0	NULL	citrate	NULL		is split into	NULL				acetate	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_4_665_s_432	16339740	The conversion involves the splitting of citrate into oxaloacetate and acetate catalyzed by citrate lyase and the decarboxylation of oxaloacetate to pyruvate and carbon dioxide catalyzed by oxaloacetate decarboxylase.	transcription
52486	3	334906	5	NULL	NULL	0	NULL	statement 1	NULL		occurs along with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_4_665_s_432	16339740	The conversion involves the splitting of citrate into oxaloacetate and acetate catalyzed by citrate lyase and the decarboxylation of oxaloacetate to pyruvate and carbon dioxide catalyzed by oxaloacetate decarboxylase.	transcription
52487	4	334906	5	NULL	NULL	0	NULL	citrate lyase	NULL		catalyzes	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_4_665_s_432	16339740	The conversion involves the splitting of citrate into oxaloacetate and acetate catalyzed by citrate lyase and the decarboxylation of oxaloacetate to pyruvate and carbon dioxide catalyzed by oxaloacetate decarboxylase.	transcription
52488	5	334906	5	NULL	NULL	0	NULL	oxaloacetate	NULL		is decarboxylatd to	NULL				pyruvate	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_4_665_s_432	16339740	The conversion involves the splitting of citrate into oxaloacetate and acetate catalyzed by citrate lyase and the decarboxylation of oxaloacetate to pyruvate and carbon dioxide catalyzed by oxaloacetate decarboxylase.	transcription
52489	6	334906	5	NULL	NULL	0	NULL	oxaloacetate	NULL		is decarboxylatd to	NULL				carbon dioxide	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_4_665_s_432	16339740	The conversion involves the splitting of citrate into oxaloacetate and acetate catalyzed by citrate lyase and the decarboxylation of oxaloacetate to pyruvate and carbon dioxide catalyzed by oxaloacetate decarboxylase.	transcription
52490	7	334906	5	NULL	NULL	0	NULL	statement 5	NULL		occurs along with	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_4_665_s_432	16339740	The conversion involves the splitting of citrate into oxaloacetate and acetate catalyzed by citrate lyase and the decarboxylation of oxaloacetate to pyruvate and carbon dioxide catalyzed by oxaloacetate decarboxylase.	transcription
52491	8	334906	5	NULL	NULL	0	NULL	oxaloacetate decarboxylase	NULL		catalyzes	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_4_665_s_432	16339740	The conversion involves the splitting of citrate into oxaloacetate and acetate catalyzed by citrate lyase and the decarboxylation of oxaloacetate to pyruvate and carbon dioxide catalyzed by oxaloacetate decarboxylase.	transcription
53736	1	334906	6	NULL	NULL	0	NULL	citrate			is converted to					oxaloacetate					NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_4_665_s_432	16339740	The conversion involves the splitting of citrate into oxaloacetate and acetate catalyzed by citrate lyase and the decarboxylation of oxaloacetate to pyruvate and carbon dioxide catalyzed by oxaloacetate decarboxylase.	transcription
53737	2	334906	6	NULL	NULL	0	NULL	citrate			is converted to					acetate					NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_4_665_s_432	16339740	The conversion involves the splitting of citrate into oxaloacetate and acetate catalyzed by citrate lyase and the decarboxylation of oxaloacetate to pyruvate and carbon dioxide catalyzed by oxaloacetate decarboxylase.	transcription
53738	3	334906	6	NULL	NULL	0	NULL	citrate lyase			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_4_665_s_432	16339740	The conversion involves the splitting of citrate into oxaloacetate and acetate catalyzed by citrate lyase and the decarboxylation of oxaloacetate to pyruvate and carbon dioxide catalyzed by oxaloacetate decarboxylase.	transcription
53740	4	334906	6	NULL	NULL	0	NULL	citrate lyase			catalyzes					statement 2					NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_4_665_s_432	16339740	The conversion involves the splitting of citrate into oxaloacetate and acetate catalyzed by citrate lyase and the decarboxylation of oxaloacetate to pyruvate and carbon dioxide catalyzed by oxaloacetate decarboxylase.	transcription
53741	5	334906	6	NULL	NULL	0	NULL	Oxaloacetate			decarboxylated to					pyruvate					NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_4_665_s_432	16339740	The conversion involves the splitting of citrate into oxaloacetate and acetate catalyzed by citrate lyase and the decarboxylation of oxaloacetate to pyruvate and carbon dioxide catalyzed by oxaloacetate decarboxylase.	transcription
53742	6	334906	6	NULL	NULL	0	NULL	Oxaloacetate			decarboxylated to					carbon dioxide					NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_4_665_s_432	16339740	The conversion involves the splitting of citrate into oxaloacetate and acetate catalyzed by citrate lyase and the decarboxylation of oxaloacetate to pyruvate and carbon dioxide catalyzed by oxaloacetate decarboxylase.	transcription
53743	7	334906	6	NULL	NULL	0	NULL	oxaloacetate decarboxylase			catalyzes					statement 5					NULL		0	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_4_665_s_432	16339740	The conversion involves the splitting of citrate into oxaloacetate and acetate catalyzed by citrate lyase and the decarboxylation of oxaloacetate to pyruvate and carbon dioxide catalyzed by oxaloacetate decarboxylase.	transcription
53744	8	334906	6	NULL	NULL	0	NULL	oxaloacetate decarboxylase			catalyzes					statement 6					NULL		NULL	NULL	NULL	NULL	gw70_microbiolmolbiolr_69_4_665_s_432	16339740	The conversion involves the splitting of citrate into oxaloacetate and acetate catalyzed by citrate lyase and the decarboxylation of oxaloacetate to pyruvate and carbon dioxide catalyzed by oxaloacetate decarboxylase.	transcription
52069	1	334907	5	NULL	NULL	0	NULL	pyruvate	NULL		is carboxylated to	NULL				oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_22_2_105_s_218	9729766	1.1) catalyzes the biotin-dependent carboxylation of  pyruvate to form oxaloacetate ( Fig. 2).	transcription
52070	2	334907	5	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				biotin	NULL				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_22_2_105_s_218	9729766	1.1) catalyzes the biotin-dependent carboxylation of  pyruvate to form oxaloacetate ( Fig. 2).	transcription
53745	1	334907	6	NULL	NULL	0	NULL	pyruvate			is carboxylated to					oxaloacetate					NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_22_2_105_s_218	9729766	1.1) catalyzes the biotin-dependent carboxylation of  pyruvate to form oxaloacetate ( Fig. 2).	transcription
53746	2	334907	6	NULL	NULL	0	NULL	statement 1			is dependent on					biotin					NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_22_2_105_s_218	9729766	1.1) catalyzes the biotin-dependent carboxylation of  pyruvate to form oxaloacetate ( Fig. 2).	transcription
52071	1	334908	5	NULL	NULL	0	NULL	CHA			is converted to					pyruvate					NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_1_41_s_178	12486039	This result indicated that LigK catalyzes the conversion of CHA to pyruvate and oxaloacetate.	transcription
52072	2	334908	5	NULL	NULL	0	NULL	LigK			is converted to					oxaloacetate					NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_185_1_41_s_178	12486039	This result indicated that LigK catalyzes the conversion of CHA to pyruvate and oxaloacetate.	transcription
54312	3	334908	5	NULL	NULL	0	NULL	statement 1			occurs along with					statement 2					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_1_41_s_178	12486039	This result indicated that LigK catalyzes the conversion of CHA to pyruvate and oxaloacetate.	transcription
54313	4	334908	5	NULL	NULL	0	NULL	LigK			catalyzes					statement 3					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_1_41_s_178	12486039	This result indicated that LigK catalyzes the conversion of CHA to pyruvate and oxaloacetate.	transcription
53747	1	334908	6	NULL	NULL	0	NULL	CHA			is converted to					pyruvate					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_1_41_s_178	12486039	This result indicated that LigK catalyzes the conversion of CHA to pyruvate and oxaloacetate.	transcription
53748	2	334908	6	NULL	NULL	0	NULL	CHA			is converted to					oxaloacetate					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_1_41_s_178	12486039	This result indicated that LigK catalyzes the conversion of CHA to pyruvate and oxaloacetate.	transcription
53749	3	334908	6	NULL	NULL	0	NULL	LigK			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_1_41_s_178	12486039	This result indicated that LigK catalyzes the conversion of CHA to pyruvate and oxaloacetate.	transcription
53750	4	334908	6	NULL	NULL	0	NULL	LigK			catalyzes					statement 2					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_1_41_s_178	12486039	This result indicated that LigK catalyzes the conversion of CHA to pyruvate and oxaloacetate.	transcription
52073	1	334909	5	NULL	NULL	0	NULL	citrate	NULL		is converted to	NULL				pyruvate	NULL				NULL	lactic acid bacteria	NULL	NULL	NULL	NULL	gw60_jbacteriol_181_14_4411_s_9	10400601	Conversion of citrate into pyruvate by lactic acid bacteria requires three enzymes: a citrate permease (CitP), a citrate lyase (CL) that cleaves intracellular citrate into acetate and oxaloacetate, and an oxaloacetate decarboxylase that catalyzes the oxaloacetate decarboxylation into carbon dioxide and pyruvate.	transcription
52074	2	334909	5	NULL	NULL	0	NULL	CitP	NULL		is required for	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_14_4411_s_9	10400601	Conversion of citrate into pyruvate by lactic acid bacteria requires three enzymes: a citrate permease (CitP), a citrate lyase (CL) that cleaves intracellular citrate into acetate and oxaloacetate, and an oxaloacetate decarboxylase that catalyzes the oxaloacetate decarboxylation into carbon dioxide and pyruvate.	transcription
52075	3	334909	5	NULL	NULL	0	NULL	CL	NULL		is required for	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_14_4411_s_9	10400601	Conversion of citrate into pyruvate by lactic acid bacteria requires three enzymes: a citrate permease (CitP), a citrate lyase (CL) that cleaves intracellular citrate into acetate and oxaloacetate, and an oxaloacetate decarboxylase that catalyzes the oxaloacetate decarboxylation into carbon dioxide and pyruvate.	transcription
52076	4	334909	5	NULL	NULL	0	NULL	oxaloacetate decarboxylase	NULL		is required for	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_14_4411_s_9	10400601	Conversion of citrate into pyruvate by lactic acid bacteria requires three enzymes: a citrate permease (CitP), a citrate lyase (CL) that cleaves intracellular citrate into acetate and oxaloacetate, and an oxaloacetate decarboxylase that catalyzes the oxaloacetate decarboxylation into carbon dioxide and pyruvate.	transcription
52077	5	334909	5	NULL	NULL	0	NULL	CitP	NULL		is	NULL				citrate permease	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_14_4411_s_9	10400601	Conversion of citrate into pyruvate by lactic acid bacteria requires three enzymes: a citrate permease (CitP), a citrate lyase (CL) that cleaves intracellular citrate into acetate and oxaloacetate, and an oxaloacetate decarboxylase that catalyzes the oxaloacetate decarboxylation into carbon dioxide and pyruvate.	transcription
52078	6	334909	5	NULL	NULL	0	NULL	CL	NULL		is	NULL				citrate lyase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_14_4411_s_9	10400601	Conversion of citrate into pyruvate by lactic acid bacteria requires three enzymes: a citrate permease (CitP), a citrate lyase (CL) that cleaves intracellular citrate into acetate and oxaloacetate, and an oxaloacetate decarboxylase that catalyzes the oxaloacetate decarboxylation into carbon dioxide and pyruvate.	transcription
52079	7	334909	5	NULL	NULL	0	NULL	citrate		intracellular	is cleaved into					acetate					NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_14_4411_s_9	10400601	Conversion of citrate into pyruvate by lactic acid bacteria requires three enzymes: a citrate permease (CitP), a citrate lyase (CL) that cleaves intracellular citrate into acetate and oxaloacetate, and an oxaloacetate decarboxylase that catalyzes the oxaloacetate decarboxylation into carbon dioxide and pyruvate.	transcription
52080	10	334909	5	NULL	NULL	0	NULL	CL			catalyzes					statement 9					NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_14_4411_s_9	10400601	Conversion of citrate into pyruvate by lactic acid bacteria requires three enzymes: a citrate permease (CitP), a citrate lyase (CL) that cleaves intracellular citrate into acetate and oxaloacetate, and an oxaloacetate decarboxylase that catalyzes the oxaloacetate decarboxylation into carbon dioxide and pyruvate.	transcription
52081	11	334909	5	NULL	NULL	0	NULL	oxaloacetate			is decarboxylatd to					carbon dioxide					NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_14_4411_s_9	10400601	Conversion of citrate into pyruvate by lactic acid bacteria requires three enzymes: a citrate permease (CitP), a citrate lyase (CL) that cleaves intracellular citrate into acetate and oxaloacetate, and an oxaloacetate decarboxylase that catalyzes the oxaloacetate decarboxylation into carbon dioxide and pyruvate.	transcription
52082	14	334909	5	NULL	NULL	0	NULL	oxaloacetate decarboxylase			catalyzes					statement 13					NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_14_4411_s_9	10400601	Conversion of citrate into pyruvate by lactic acid bacteria requires three enzymes: a citrate permease (CitP), a citrate lyase (CL) that cleaves intracellular citrate into acetate and oxaloacetate, and an oxaloacetate decarboxylase that catalyzes the oxaloacetate decarboxylation into carbon dioxide and pyruvate.	transcription
54314	8	334909	5	NULL	NULL	0	NULL	citrate		intracellular	is cleaved into					oxaloacetate					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_14_4411_s_9	10400601	Conversion of citrate into pyruvate by lactic acid bacteria requires three enzymes: a citrate permease (CitP), a citrate lyase (CL) that cleaves intracellular citrate into acetate and oxaloacetate, and an oxaloacetate decarboxylase that catalyzes the oxaloacetate decarboxylation into carbon dioxide and pyruvate.	transcription
54315	9	334909	5	NULL	NULL	0	NULL	statement 7			occurs along with					statement 8					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_14_4411_s_9	10400601	Conversion of citrate into pyruvate by lactic acid bacteria requires three enzymes: a citrate permease (CitP), a citrate lyase (CL) that cleaves intracellular citrate into acetate and oxaloacetate, and an oxaloacetate decarboxylase that catalyzes the oxaloacetate decarboxylation into carbon dioxide and pyruvate.	transcription
54316	12	334909	5	NULL	NULL	0	NULL	oxaloacetate			is decarboxylatd to					pyruvate					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_14_4411_s_9	10400601	Conversion of citrate into pyruvate by lactic acid bacteria requires three enzymes: a citrate permease (CitP), a citrate lyase (CL) that cleaves intracellular citrate into acetate and oxaloacetate, and an oxaloacetate decarboxylase that catalyzes the oxaloacetate decarboxylation into carbon dioxide and pyruvate.	transcription
54317	13	334909	5	NULL	NULL	0	NULL	statement 11			occurs along with					statement 12					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_14_4411_s_9	10400601	Conversion of citrate into pyruvate by lactic acid bacteria requires three enzymes: a citrate permease (CitP), a citrate lyase (CL) that cleaves intracellular citrate into acetate and oxaloacetate, and an oxaloacetate decarboxylase that catalyzes the oxaloacetate decarboxylation into carbon dioxide and pyruvate.	transcription
53751	1	334909	6	NULL	NULL	0	NULL	citrate			is converted to					pyruvate					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_14_4411_s_9	10400601	Conversion of citrate into pyruvate by lactic acid bacteria requires three enzymes: a citrate permease (CitP), a citrate lyase (CL) that cleaves intracellular citrate into acetate and oxaloacetate, and an oxaloacetate decarboxylase that catalyzes the oxaloacetate decarboxylation into carbon dioxide and pyruvate.	transcription
53752	2	334909	6	NULL	NULL	0	NULL	lactic acid bacteria			performs					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_14_4411_s_9	10400601	Conversion of citrate into pyruvate by lactic acid bacteria requires three enzymes: a citrate permease (CitP), a citrate lyase (CL) that cleaves intracellular citrate into acetate and oxaloacetate, and an oxaloacetate decarboxylase that catalyzes the oxaloacetate decarboxylation into carbon dioxide and pyruvate.	transcription
53753	3	334909	6	NULL	NULL	0	NULL	statement 1			requires					CitP					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_14_4411_s_9	10400601	Conversion of citrate into pyruvate by lactic acid bacteria requires three enzymes: a citrate permease (CitP), a citrate lyase (CL) that cleaves intracellular citrate into acetate and oxaloacetate, and an oxaloacetate decarboxylase that catalyzes the oxaloacetate decarboxylation into carbon dioxide and pyruvate.	transcription
53754	4	334909	6	NULL	NULL	0	NULL	statement 1			requires					CL					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_14_4411_s_9	10400601	Conversion of citrate into pyruvate by lactic acid bacteria requires three enzymes: a citrate permease (CitP), a citrate lyase (CL) that cleaves intracellular citrate into acetate and oxaloacetate, and an oxaloacetate decarboxylase that catalyzes the oxaloacetate decarboxylation into carbon dioxide and pyruvate.	transcription
53755	5	334909	6	NULL	NULL	0	NULL	statement 1			requires					oxaloacetate decarboxylase					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_14_4411_s_9	10400601	Conversion of citrate into pyruvate by lactic acid bacteria requires three enzymes: a citrate permease (CitP), a citrate lyase (CL) that cleaves intracellular citrate into acetate and oxaloacetate, and an oxaloacetate decarboxylase that catalyzes the oxaloacetate decarboxylation into carbon dioxide and pyruvate.	transcription
53756	6	334909	6	NULL	NULL	0	NULL	CitP			is					citrate permease					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_14_4411_s_9	10400601	Conversion of citrate into pyruvate by lactic acid bacteria requires three enzymes: a citrate permease (CitP), a citrate lyase (CL) that cleaves intracellular citrate into acetate and oxaloacetate, and an oxaloacetate decarboxylase that catalyzes the oxaloacetate decarboxylation into carbon dioxide and pyruvate.	transcription
53757	7	334909	6	NULL	NULL	0	NULL	CL			is					citrate lyase					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_14_4411_s_9	10400601	Conversion of citrate into pyruvate by lactic acid bacteria requires three enzymes: a citrate permease (CitP), a citrate lyase (CL) that cleaves intracellular citrate into acetate and oxaloacetate, and an oxaloacetate decarboxylase that catalyzes the oxaloacetate decarboxylation into carbon dioxide and pyruvate.	transcription
53758	8	334909	6	NULL	NULL	0	NULL	citrate		intracellular	is cleaved into					acetate					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_14_4411_s_9	10400601	Conversion of citrate into pyruvate by lactic acid bacteria requires three enzymes: a citrate permease (CitP), a citrate lyase (CL) that cleaves intracellular citrate into acetate and oxaloacetate, and an oxaloacetate decarboxylase that catalyzes the oxaloacetate decarboxylation into carbon dioxide and pyruvate.	transcription
53759	9	334909	6	NULL	NULL	0	NULL	citrate		intracellular	is cleaved into					oxaloacetate					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_14_4411_s_9	10400601	Conversion of citrate into pyruvate by lactic acid bacteria requires three enzymes: a citrate permease (CitP), a citrate lyase (CL) that cleaves intracellular citrate into acetate and oxaloacetate, and an oxaloacetate decarboxylase that catalyzes the oxaloacetate decarboxylation into carbon dioxide and pyruvate.	transcription
53760	10	334909	6	NULL	NULL	0	NULL	CL			catalyzes					statement 8					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_14_4411_s_9	10400601	Conversion of citrate into pyruvate by lactic acid bacteria requires three enzymes: a citrate permease (CitP), a citrate lyase (CL) that cleaves intracellular citrate into acetate and oxaloacetate, and an oxaloacetate decarboxylase that catalyzes the oxaloacetate decarboxylation into carbon dioxide and pyruvate.	transcription
53761	11	334909	6	NULL	NULL	0	NULL	CL			catalyzes					statement 9					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_14_4411_s_9	10400601	Conversion of citrate into pyruvate by lactic acid bacteria requires three enzymes: a citrate permease (CitP), a citrate lyase (CL) that cleaves intracellular citrate into acetate and oxaloacetate, and an oxaloacetate decarboxylase that catalyzes the oxaloacetate decarboxylation into carbon dioxide and pyruvate.	transcription
53762	12	334909	6	NULL	NULL	0	NULL	Oxaloacetate			is decarboxylated into					carbon dioxide					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_14_4411_s_9	10400601	Conversion of citrate into pyruvate by lactic acid bacteria requires three enzymes: a citrate permease (CitP), a citrate lyase (CL) that cleaves intracellular citrate into acetate and oxaloacetate, and an oxaloacetate decarboxylase that catalyzes the oxaloacetate decarboxylation into carbon dioxide and pyruvate.	transcription
53763	13	334909	6	NULL	NULL	0	NULL	oxaloacetate			is decarboxylated into					pyruvate					NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_14_4411_s_9	10400601	Conversion of citrate into pyruvate by lactic acid bacteria requires three enzymes: a citrate permease (CitP), a citrate lyase (CL) that cleaves intracellular citrate into acetate and oxaloacetate, and an oxaloacetate decarboxylase that catalyzes the oxaloacetate decarboxylation into carbon dioxide and pyruvate.	transcription
53764	14	334909	6	NULL	NULL	0	NULL	oxaloacetate decarboxylase			catalyzes					statement 12					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_14_4411_s_9	10400601	Conversion of citrate into pyruvate by lactic acid bacteria requires three enzymes: a citrate permease (CitP), a citrate lyase (CL) that cleaves intracellular citrate into acetate and oxaloacetate, and an oxaloacetate decarboxylase that catalyzes the oxaloacetate decarboxylation into carbon dioxide and pyruvate.	transcription
53765	15	334909	6	NULL	NULL	0	NULL	oxaloacetate decarboxylase			catalyzes					statement 13					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_14_4411_s_9	10400601	Conversion of citrate into pyruvate by lactic acid bacteria requires three enzymes: a citrate permease (CitP), a citrate lyase (CL) that cleaves intracellular citrate into acetate and oxaloacetate, and an oxaloacetate decarboxylase that catalyzes the oxaloacetate decarboxylation into carbon dioxide and pyruvate.	transcription
52083	1	334910	5	NULL	NULL	0	NULL	pyruvate	NULL		is converted to	NULL				oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevphysiol_65_0_401_s_142	12524459	Glutamate lost to the system by oxidation is replaced through anaplerosis, beginning  with pyruvate carboxylase catalyzed conversion of pyruvate to oxaloacetate.	transcription
52084	2	334910	5	NULL	NULL	0	NULL	pyruvate carboxylase	NULL		catalyzes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevphysiol_65_0_401_s_142	12524459	Glutamate lost to the system by oxidation is replaced through anaplerosis, beginning  with pyruvate carboxylase catalyzed conversion of pyruvate to oxaloacetate.	transcription
52085	3	334910	5	NULL	NULL	0	NULL	glutamate	NULL	loss of	is caused by	NULL				oxidation	NULL				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_65_0_401_s_142	12524459	Glutamate lost to the system by oxidation is replaced through anaplerosis, beginning  with pyruvate carboxylase catalyzed conversion of pyruvate to oxaloacetate.	transcription
52087	5	334910	5	NULL	NULL	0	NULL	anaplerosis	NULL		replaces	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_annurevphysiol_65_0_401_s_142	12524459	Glutamate lost to the system by oxidation is replaced through anaplerosis, beginning  with pyruvate carboxylase catalyzed conversion of pyruvate to oxaloacetate.	transcription
53766	1	334910	6	NULL	NULL	0	NULL	pyruvate			is converted to					oxaloacetate					NULL		0	NULL	NULL	NULL	gw70_annurevphysiol_65_0_401_s_142	12524459	Glutamate lost to the system by oxidation is replaced through anaplerosis, beginning  with pyruvate carboxylase catalyzed conversion of pyruvate to oxaloacetate.	transcription
53767	2	334910	6	NULL	NULL	0	NULL	pyruvate carboxylase			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw70_annurevphysiol_65_0_401_s_142	12524459	Glutamate lost to the system by oxidation is replaced through anaplerosis, beginning  with pyruvate carboxylase catalyzed conversion of pyruvate to oxaloacetate.	transcription
53768	3	334910	6	NULL	NULL	0	NULL	glutamate		lost	is replaced through					anaplerosis					NULL		0	NULL	NULL	NULL	gw70_annurevphysiol_65_0_401_s_142	12524459	Glutamate lost to the system by oxidation is replaced through anaplerosis, beginning  with pyruvate carboxylase catalyzed conversion of pyruvate to oxaloacetate.	transcription
52088	1	334911	5	NULL	NULL	0	NULL	B. subtilis	NULL		contains	NULL				PC	NULL				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_7_3986_s_33	12839772	B. subtilis contains a pyruvate carboxylase (PC), encoded by  pycA, to convert pyruvate to oxaloacetate, and lacks phosphoenolpyruvate carboxylase activity ( ).	transcription
52089	2	334911	5	NULL	NULL	0	NULL	PC	NULL		is	NULL				pyruvate carboxylase	NULL				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_7_3986_s_33	12839772	B. subtilis contains a pyruvate carboxylase (PC), encoded by  pycA, to convert pyruvate to oxaloacetate, and lacks phosphoenolpyruvate carboxylase activity ( ).	transcription
52090	3	334911	5	NULL	NULL	0	NULL	PC	NULL		is encoded by	NULL				pycA	NULL				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_7_3986_s_33	12839772	B. subtilis contains a pyruvate carboxylase (PC), encoded by  pycA, to convert pyruvate to oxaloacetate, and lacks phosphoenolpyruvate carboxylase activity ( ).	transcription
52091	4	334911	5	NULL	NULL	0	NULL	pyruvate	NULL		is converted to	NULL				oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_7_3986_s_33	12839772	B. subtilis contains a pyruvate carboxylase (PC), encoded by  pycA, to convert pyruvate to oxaloacetate, and lacks phosphoenolpyruvate carboxylase activity ( ).	transcription
52092	5	334911	5	NULL	NULL	0	NULL	PC	NULL		catalyzes	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_7_3986_s_33	12839772	B. subtilis contains a pyruvate carboxylase (PC), encoded by  pycA, to convert pyruvate to oxaloacetate, and lacks phosphoenolpyruvate carboxylase activity ( ).	transcription
52093	6	334911	5	NULL	NULL	0	NULL	PC	NULL		lacks	NULL				phosphoenolpyruvate carboxylase activity	NULL				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_7_3986_s_33	12839772	B. subtilis contains a pyruvate carboxylase (PC), encoded by  pycA, to convert pyruvate to oxaloacetate, and lacks phosphoenolpyruvate carboxylase activity ( ).	transcription
53769	1	334911	6	NULL	NULL	0	NULL	PC			is					pyruvate carboxylase					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_7_3986_s_33	12839772	B. subtilis contains a pyruvate carboxylase (PC), encoded by  pycA, to convert pyruvate to oxaloacetate, and lacks phosphoenolpyruvate carboxylase activity ( ).	transcription
53770	2	334911	6	NULL	NULL	0	NULL	pyruvate			is converted to					oxaloacetate					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_7_3986_s_33	12839772	B. subtilis contains a pyruvate carboxylase (PC), encoded by  pycA, to convert pyruvate to oxaloacetate, and lacks phosphoenolpyruvate carboxylase activity ( ).	transcription
53771	3	334911	6	NULL	NULL	0	NULL	PC			catalyzes					statement 2					NULL		NULL	NULL	NULL	NULL	gw70_applenvironmicrob_69_7_3986_s_33	12839772	B. subtilis contains a pyruvate carboxylase (PC), encoded by  pycA, to convert pyruvate to oxaloacetate, and lacks phosphoenolpyruvate carboxylase activity ( ).	transcription
53772	4	334911	6	NULL	NULL	0	NULL	PC			lacks					phosphoenolpyruvate carboxylase		activity of 			NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_7_3986_s_33	12839772	B. subtilis contains a pyruvate carboxylase (PC), encoded by  pycA, to convert pyruvate to oxaloacetate, and lacks phosphoenolpyruvate carboxylase activity ( ).	transcription
53773	5	334911	6	NULL	NULL	0	NULL	PC			is encoded by					pycA					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_7_3986_s_33	12839772	B. subtilis contains a pyruvate carboxylase (PC), encoded by  pycA, to convert pyruvate to oxaloacetate, and lacks phosphoenolpyruvate carboxylase activity ( ).	transcription
53774	6	334911	6	NULL	NULL	0	NULL	B. subtilis			contains					PC					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_7_3986_s_33	12839772	B. subtilis contains a pyruvate carboxylase (PC), encoded by  pycA, to convert pyruvate to oxaloacetate, and lacks phosphoenolpyruvate carboxylase activity ( ).	transcription
52094	1	334912	5	NULL	NULL	0	NULL	PycA	NULL		is	NULL				pyruvate carboxylase	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_24_8478_s_281	15576798	Pyruvate carboxylase (PycA) catalyzes the ATP-dependent carboxylation of pyruvate to form oxaloacetate, a substrate for aspartate aminotransferase (AspB).	transcription
52095	2	334912	5	NULL	NULL	0	NULL	pyruvate	NULL		is carboxylated to	NULL				oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_24_8478_s_281	15576798	Pyruvate carboxylase (PycA) catalyzes the ATP-dependent carboxylation of pyruvate to form oxaloacetate, a substrate for aspartate aminotransferase (AspB).	transcription
52096	3	334912	5	NULL	NULL	0	NULL	statement 2	NULL		is dependent on	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_24_8478_s_281	15576798	Pyruvate carboxylase (PycA) catalyzes the ATP-dependent carboxylation of pyruvate to form oxaloacetate, a substrate for aspartate aminotransferase (AspB).	transcription
52097	4	334912	5	NULL	NULL	0	NULL	PycA	NULL		catalyzes	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_24_8478_s_281	15576798	Pyruvate carboxylase (PycA) catalyzes the ATP-dependent carboxylation of pyruvate to form oxaloacetate, a substrate for aspartate aminotransferase (AspB).	transcription
52098	5	334912	5	NULL	NULL	0	NULL	oxaloacetate	NULL		is a substrate for	NULL				AspB	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_24_8478_s_281	15576798	Pyruvate carboxylase (PycA) catalyzes the ATP-dependent carboxylation of pyruvate to form oxaloacetate, a substrate for aspartate aminotransferase (AspB).	transcription
52099	6	334912	5	NULL	NULL	0	NULL	AspB	NULL		is	NULL				aspartate aminotransferase	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_24_8478_s_281	15576798	Pyruvate carboxylase (PycA) catalyzes the ATP-dependent carboxylation of pyruvate to form oxaloacetate, a substrate for aspartate aminotransferase (AspB).	transcription
53784	1	334912	6	NULL	NULL	0	NULL	pyruvate			is carboxylated to					oxaloacetate					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_24_8478_s_281	15576798	Pyruvate carboxylase (PycA) catalyzes the ATP-dependent carboxylation of pyruvate to form oxaloacetate, a substrate for aspartate aminotransferase (AspB).	transcription
53785	2	334912	6	NULL	NULL	0	NULL	statement 1			is dependent on					ATP					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_24_8478_s_281	15576798	Pyruvate carboxylase (PycA) catalyzes the ATP-dependent carboxylation of pyruvate to form oxaloacetate, a substrate for aspartate aminotransferase (AspB).	transcription
53786	3	334912	6	NULL	NULL	0	NULL	PycA			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_24_8478_s_281	15576798	Pyruvate carboxylase (PycA) catalyzes the ATP-dependent carboxylation of pyruvate to form oxaloacetate, a substrate for aspartate aminotransferase (AspB).	transcription
53787	4	334912	6	NULL	NULL	0	NULL	PycA			is					Pyruvate carboxylase					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_24_8478_s_281	15576798	Pyruvate carboxylase (PycA) catalyzes the ATP-dependent carboxylation of pyruvate to form oxaloacetate, a substrate for aspartate aminotransferase (AspB).	transcription
53788	5	334912	6	NULL	NULL	0	NULL	Oxaloacetate			is a substrate for					aspartate aminotransferase 					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_24_8478_s_281	15576798	Pyruvate carboxylase (PycA) catalyzes the ATP-dependent carboxylation of pyruvate to form oxaloacetate, a substrate for aspartate aminotransferase (AspB).	transcription
53789	6	334912	6	NULL	NULL	0	NULL	AspB			is					aspartate aminotransferase					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_24_8478_s_281	15576798	Pyruvate carboxylase (PycA) catalyzes the ATP-dependent carboxylation of pyruvate to form oxaloacetate, a substrate for aspartate aminotransferase (AspB).	transcription
52100	1	334913	5	NULL	NULL	0	NULL	PC	NULL		is	NULL				pyruvate carboxylase	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_27466_s_22	15917242	Pyruvate carboxylase (PC), a member of the biotin-containing enzyme family, catalyzes the ATP-dependent carboxylation of pyruvate to oxaloacetate ( ).	transcription
52101	2	334913	5	NULL	NULL	0	NULL	PC	NULL		is a member of	NULL				biotin-containing enzyme family	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_27466_s_22	15917242	Pyruvate carboxylase (PC), a member of the biotin-containing enzyme family, catalyzes the ATP-dependent carboxylation of pyruvate to oxaloacetate ( ).	transcription
52102	3	334913	5	NULL	NULL	0	NULL	pyruvate	NULL		is carboxylated to	NULL				oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_27466_s_22	15917242	Pyruvate carboxylase (PC), a member of the biotin-containing enzyme family, catalyzes the ATP-dependent carboxylation of pyruvate to oxaloacetate ( ).	transcription
52103	4	334913	5	NULL	NULL	0	NULL	statement 3	NULL		is dependent on	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_27466_s_22	15917242	Pyruvate carboxylase (PC), a member of the biotin-containing enzyme family, catalyzes the ATP-dependent carboxylation of pyruvate to oxaloacetate ( ).	transcription
52104	5	334913	5	NULL	NULL	0	NULL	PC	NULL		catalyzes	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_27466_s_22	15917242	Pyruvate carboxylase (PC), a member of the biotin-containing enzyme family, catalyzes the ATP-dependent carboxylation of pyruvate to oxaloacetate ( ).	transcription
53790	1	334913	6	NULL	NULL	0	NULL	PC			is					pyruvate carboxylase					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_27466_s_22	15917242	Pyruvate carboxylase (PC), a member of the biotin-containing enzyme family, catalyzes the ATP-dependent carboxylation of pyruvate to oxaloacetate ( ).	transcription
53791	2	334913	6	NULL	NULL	0	NULL	PC			is a member of					biotin-containing enzyme family					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_27466_s_22	15917242	Pyruvate carboxylase (PC), a member of the biotin-containing enzyme family, catalyzes the ATP-dependent carboxylation of pyruvate to oxaloacetate ( ).	transcription
53792	3	334913	6	NULL	NULL	0	NULL	pyruvate			is carboxylated to					oxaloacetate					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_27466_s_22	15917242	Pyruvate carboxylase (PC), a member of the biotin-containing enzyme family, catalyzes the ATP-dependent carboxylation of pyruvate to oxaloacetate ( ).	transcription
53793	4	334913	6	NULL	NULL	0	NULL	statement 3			is dependent on					ATP					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_27466_s_22	15917242	Pyruvate carboxylase (PC), a member of the biotin-containing enzyme family, catalyzes the ATP-dependent carboxylation of pyruvate to oxaloacetate ( ).	transcription
53794	5	334913	6	NULL	NULL	0	NULL	PC			catalyzes					statement 3					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_27466_s_22	15917242	Pyruvate carboxylase (PC), a member of the biotin-containing enzyme family, catalyzes the ATP-dependent carboxylation of pyruvate to oxaloacetate ( ).	transcription
52105	1	334914	5	NULL	NULL	0	NULL	oxaloacetate	NULL		is formed from	NULL				pyruvate & HCO3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_30_27176_s_21	11986306	Pyruvate carboxylase catalyzes the ATP-driven formation of oxaloacetate from pyruvate and HCO3  and P-enolpyruvate carboxykinase (PEPCK) (EC 4.1.	transcription
52106	2	334914	5	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_30_27176_s_21	11986306	Pyruvate carboxylase catalyzes the ATP-driven formation of oxaloacetate from pyruvate and HCO3  and P-enolpyruvate carboxykinase (PEPCK) (EC 4.1.	transcription
52107	3	334914	5	NULL	NULL	0	NULL	pyruvate carboxylase	NULL		catalyzes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_30_27176_s_21	11986306	Pyruvate carboxylase catalyzes the ATP-driven formation of oxaloacetate from pyruvate and HCO3  and P-enolpyruvate carboxykinase (PEPCK) (EC 4.1.	transcription
53795	1	334914	6	NULL	NULL	0	NULL	oxaloacetate			is formed from					pyruvate					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_30_27176_s_21	11986306	Pyruvate carboxylase catalyzes the ATP-driven formation of oxaloacetate from pyruvate and HCO3  and P-enolpyruvate carboxykinase (PEPCK) (EC 4.1.	transcription
53796	2	334914	6	NULL	NULL	0	NULL	Oxaloacetate			is formed from					HCO3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_30_27176_s_21	11986306	Pyruvate carboxylase catalyzes the ATP-driven formation of oxaloacetate from pyruvate and HCO3  and P-enolpyruvate carboxykinase (PEPCK) (EC 4.1.	transcription
53797	3	334914	6	NULL	NULL	0	NULL	oxaloacetate			is formed from					PEPCK					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_30_27176_s_21	11986306	Pyruvate carboxylase catalyzes the ATP-driven formation of oxaloacetate from pyruvate and HCO3  and P-enolpyruvate carboxykinase (PEPCK) (EC 4.1.	transcription
53798	4	334914	6	NULL	NULL	0	NULL	PEPCK			is					P-enolpyruvate carboxykinase					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_30_27176_s_21	11986306	Pyruvate carboxylase catalyzes the ATP-driven formation of oxaloacetate from pyruvate and HCO3  and P-enolpyruvate carboxykinase (PEPCK) (EC 4.1.	transcription
53799	5	334914	6	NULL	NULL	0	NULL	statement 1			occurs simultaneously with					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_30_27176_s_21	11986306	Pyruvate carboxylase catalyzes the ATP-driven formation of oxaloacetate from pyruvate and HCO3  and P-enolpyruvate carboxykinase (PEPCK) (EC 4.1.	transcription
53809	6	334914	6	NULL	NULL	0	NULL	statement 2			occurs simultaneously with					statement 3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_30_27176_s_21	11986306	Pyruvate carboxylase catalyzes the ATP-driven formation of oxaloacetate from pyruvate and HCO3  and P-enolpyruvate carboxykinase (PEPCK) (EC 4.1.	transcription
53810	7	334914	6	NULL	NULL	0	NULL	Pyruvate carboxylase			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_30_27176_s_21	11986306	Pyruvate carboxylase catalyzes the ATP-driven formation of oxaloacetate from pyruvate and HCO3  and P-enolpyruvate carboxykinase (PEPCK) (EC 4.1.	transcription
53811	8	334914	6	NULL	NULL	0	NULL	Pyruvate carboxylase			catalyzes					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_30_27176_s_21	11986306	Pyruvate carboxylase catalyzes the ATP-driven formation of oxaloacetate from pyruvate and HCO3  and P-enolpyruvate carboxykinase (PEPCK) (EC 4.1.	transcription
53812	9	334914	6	NULL	NULL	0	NULL	Pyruvate carboxylase			catalyzes					statement 3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_30_27176_s_21	11986306	Pyruvate carboxylase catalyzes the ATP-driven formation of oxaloacetate from pyruvate and HCO3  and P-enolpyruvate carboxykinase (PEPCK) (EC 4.1.	transcription
53813	10	334914	6	NULL	NULL	0	NULL	statement 1			is dependent on					ATP					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_30_27176_s_21	11986306	Pyruvate carboxylase catalyzes the ATP-driven formation of oxaloacetate from pyruvate and HCO3  and P-enolpyruvate carboxykinase (PEPCK) (EC 4.1.	transcription
53814	11	334914	6	NULL	NULL	0	NULL	statement 2			is dependent on					ATP					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_30_27176_s_21	11986306	Pyruvate carboxylase catalyzes the ATP-driven formation of oxaloacetate from pyruvate and HCO3  and P-enolpyruvate carboxykinase (PEPCK) (EC 4.1.	transcription
53815	12	334914	6	NULL	NULL	0	NULL	statement 3			is dependent on					ATP					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_30_27176_s_21	11986306	Pyruvate carboxylase catalyzes the ATP-driven formation of oxaloacetate from pyruvate and HCO3  and P-enolpyruvate carboxykinase (PEPCK) (EC 4.1.	transcription
52108	1	334915	5	NULL	NULL	0	NULL	oxaloacetate	NULL		is converted to	NULL				pyruvate	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_1_443_s_157	11756688	Similarly, conversion of oxaloacetate to pyruvate can be catalyzed by NADP-dependent malic enzyme and by pyruvate carboxylase.	transcription
52109	2	334915	5	NULL	NULL	0	NULL	malic enzyme	NULL		catalyzes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_1_443_s_157	11756688	Similarly, conversion of oxaloacetate to pyruvate can be catalyzed by NADP-dependent malic enzyme and by pyruvate carboxylase.	transcription
52110	3	334915	5	NULL	NULL	0	NULL	malic enzyme	NULL		is dependent on	NULL				NADP	NULL				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_1_443_s_157	11756688	Similarly, conversion of oxaloacetate to pyruvate can be catalyzed by NADP-dependent malic enzyme and by pyruvate carboxylase.	transcription
52111	4	334915	5	NULL	NULL	0	NULL	pyruvate carboxylase	NULL		catalyzes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_1_443_s_157	11756688	Similarly, conversion of oxaloacetate to pyruvate can be catalyzed by NADP-dependent malic enzyme and by pyruvate carboxylase.	transcription
53816	1	334915	6	NULL	NULL	0	NULL	oxaloacetate			is converted to					pyruvate					NULL		0	NULL	NULL	NULL	gw60_pnas_99_1_443_s_157	11756688	Similarly, conversion of oxaloacetate to pyruvate can be catalyzed by NADP-dependent malic enzyme and by pyruvate carboxylase.	transcription
53817	2	334915	6	NULL	NULL	0	NULL	malic enzyme			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw60_pnas_99_1_443_s_157	11756688	Similarly, conversion of oxaloacetate to pyruvate can be catalyzed by NADP-dependent malic enzyme and by pyruvate carboxylase.	transcription
53818	3	334915	6	NULL	NULL	0	NULL	malic enzyme			is dependent on					NADP					NULL		0	NULL	NULL	NULL	gw60_pnas_99_1_443_s_157	11756688	Similarly, conversion of oxaloacetate to pyruvate can be catalyzed by NADP-dependent malic enzyme and by pyruvate carboxylase.	transcription
53819	4	334915	6	NULL	NULL	0	NULL	pyruvate carboxylase			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw60_pnas_99_1_443_s_157	11756688	Similarly, conversion of oxaloacetate to pyruvate can be catalyzed by NADP-dependent malic enzyme and by pyruvate carboxylase.	transcription
52138	1	334916	5	NULL	NULL	0	NULL	pyruvate	NULL		is carboxylated to	NULL				oxaloacetate	NULL				NULL	B. subtilis	0	NULL	NULL	NULL	gw70_applenvironmicrob_69_7_3986_s_242	12839772	In  B. subtilis ( ,  ), the major route for aspartate synthesis involves the carboxylation of pyruvate to oxaloacetate by PC and subsequent transamination to aspartate catalyzed by glutamate:oxaloacetate transaminase.	transcription
52139	2	334916	5	NULL	NULL	0	NULL	PC	NULL		catalyzes	NULL				statement 1	NULL				NULL	B. subtilis	NULL	NULL	NULL	NULL	gw70_applenvironmicrob_69_7_3986_s_242	12839772	In  B. subtilis ( ,  ), the major route for aspartate synthesis involves the carboxylation of pyruvate to oxaloacetate by PC and subsequent transamination to aspartate catalyzed by glutamate:oxaloacetate transaminase.	transcription
52140	3	334916	5	NULL	NULL	0	NULL	oxaloacetate	NULL		is transaminated to	NULL				aspartate	NULL				NULL	B. subtilis	NULL	NULL	NULL	NULL	gw70_applenvironmicrob_69_7_3986_s_242	12839772	In  B. subtilis ( ,  ), the major route for aspartate synthesis involves the carboxylation of pyruvate to oxaloacetate by PC and subsequent transamination to aspartate catalyzed by glutamate:oxaloacetate transaminase.	transcription
52141	4	334916	5	NULL	NULL	0	NULL	glutamate:oxaloacetate transaminase	NULL		catalyzes	NULL				statement 3	NULL				NULL	B. subtilis	NULL	NULL	NULL	NULL	gw70_applenvironmicrob_69_7_3986_s_242	12839772	In  B. subtilis ( ,  ), the major route for aspartate synthesis involves the carboxylation of pyruvate to oxaloacetate by PC and subsequent transamination to aspartate catalyzed by glutamate:oxaloacetate transaminase.	transcription
53820	1	334916	6	NULL	NULL	0	NULL	pyruvate			is carboxylated to					oxaloacetate					NULL		NULL	NULL	NULL	NULL	gw70_applenvironmicrob_69_7_3986_s_242	12839772	In  B. subtilis ( ,  ), the major route for aspartate synthesis involves the carboxylation of pyruvate to oxaloacetate by PC and subsequent transamination to aspartate catalyzed by glutamate:oxaloacetate transaminase.	transcription
53821	2	334916	6	NULL	NULL	0	NULL	PC			performs					statement 1					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_7_3986_s_242	12839772	In  B. subtilis ( ,  ), the major route for aspartate synthesis involves the carboxylation of pyruvate to oxaloacetate by PC and subsequent transamination to aspartate catalyzed by glutamate:oxaloacetate transaminase.	transcription
53822	3	334916	6	NULL	NULL	0	NULL	pyruvate			is converted to					aspartate					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_7_3986_s_242	12839772	In  B. subtilis ( ,  ), the major route for aspartate synthesis involves the carboxylation of pyruvate to oxaloacetate by PC and subsequent transamination to aspartate catalyzed by glutamate:oxaloacetate transaminase.	transcription
53823	4	334916	6	NULL	NULL	0	NULL	glutamate:oxaloacetate transaminase			catalyzes					statement 3					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_7_3986_s_242	12839772	In  B. subtilis ( ,  ), the major route for aspartate synthesis involves the carboxylation of pyruvate to oxaloacetate by PC and subsequent transamination to aspartate catalyzed by glutamate:oxaloacetate transaminase.	transcription
52142	1	334917	5	NULL	NULL	0	NULL	PC	NULL		is	NULL				pyruvate carboxylase	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_314_3_824_s_93	14741710	Biotin is the cofactor of pyruvate carboxylase (PC), which catalyzes pyruvate to oxaloacetate,  and acetyl CoA carboxylase (ACC), which catalyzes acetyl CoA to malonyl CoA.	transcription
52143	2	334917	5	NULL	NULL	0	NULL	biotin	NULL		is a cofactor of	NULL				PC	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_314_3_824_s_93	14741710	Biotin is the cofactor of pyruvate carboxylase (PC), which catalyzes pyruvate to oxaloacetate,  and acetyl CoA carboxylase (ACC), which catalyzes acetyl CoA to malonyl CoA.	transcription
52144	3	334917	5	NULL	NULL	0	NULL	pyruvate	NULL		is converted to	NULL				oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_314_3_824_s_93	14741710	Biotin is the cofactor of pyruvate carboxylase (PC), which catalyzes pyruvate to oxaloacetate,  and acetyl CoA carboxylase (ACC), which catalyzes acetyl CoA to malonyl CoA.	transcription
52145	4	334917	5	NULL	NULL	0	NULL	ACC	NULL		is	NULL				acetyl CoA carboxylase	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_314_3_824_s_93	14741710	Biotin is the cofactor of pyruvate carboxylase (PC), which catalyzes pyruvate to oxaloacetate,  and acetyl CoA carboxylase (ACC), which catalyzes acetyl CoA to malonyl CoA.	transcription
52146	5	334917	5	NULL	NULL	0	NULL	biotin	NULL		is a cofactor of	NULL				ACC	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_314_3_824_s_93	14741710	Biotin is the cofactor of pyruvate carboxylase (PC), which catalyzes pyruvate to oxaloacetate,  and acetyl CoA carboxylase (ACC), which catalyzes acetyl CoA to malonyl CoA.	transcription
52147	6	334917	5	NULL	NULL	0	NULL	acetyl CoA	NULL		is converted to	NULL				malonyl CoA	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_314_3_824_s_93	14741710	Biotin is the cofactor of pyruvate carboxylase (PC), which catalyzes pyruvate to oxaloacetate,  and acetyl CoA carboxylase (ACC), which catalyzes acetyl CoA to malonyl CoA.	transcription
52148	7	334917	5	NULL	NULL	0	NULL	ACC	NULL		catalyzes	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_314_3_824_s_93	14741710	Biotin is the cofactor of pyruvate carboxylase (PC), which catalyzes pyruvate to oxaloacetate,  and acetyl CoA carboxylase (ACC), which catalyzes acetyl CoA to malonyl CoA.	transcription
53824	1	334917	6	NULL	NULL	0	NULL	PC			is					pyruvate carboxylase					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_314_3_824_s_93	14741710	Biotin is the cofactor of pyruvate carboxylase (PC), which catalyzes pyruvate to oxaloacetate,  and acetyl CoA carboxylase (ACC), which catalyzes acetyl CoA to malonyl CoA.	transcription
53825	2	334917	6	NULL	NULL	0	NULL	biotin			is cofactor of					PC					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_314_3_824_s_93	14741710	Biotin is the cofactor of pyruvate carboxylase (PC), which catalyzes pyruvate to oxaloacetate,  and acetyl CoA carboxylase (ACC), which catalyzes acetyl CoA to malonyl CoA.	transcription
53826	3	334917	6	NULL	NULL	0	NULL	pyruvate			is converted to					oxaloacetate					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_314_3_824_s_93	14741710	Biotin is the cofactor of pyruvate carboxylase (PC), which catalyzes pyruvate to oxaloacetate,  and acetyl CoA carboxylase (ACC), which catalyzes acetyl CoA to malonyl CoA.	transcription
53827	4	334917	6	NULL	NULL	0	NULL	ACC			is					acetyl CoA carboxylase					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_314_3_824_s_93	14741710	Biotin is the cofactor of pyruvate carboxylase (PC), which catalyzes pyruvate to oxaloacetate,  and acetyl CoA carboxylase (ACC), which catalyzes acetyl CoA to malonyl CoA.	transcription
53828	5	334917	6	NULL	NULL	0	NULL	acetyl CoA			is converted to					malonyl CoA					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_314_3_824_s_93	14741710	Biotin is the cofactor of pyruvate carboxylase (PC), which catalyzes pyruvate to oxaloacetate,  and acetyl CoA carboxylase (ACC), which catalyzes acetyl CoA to malonyl CoA.	transcription
53829	6	334917	6	NULL	NULL	0	NULL	ACC			catalyzes					statement 5					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_314_3_824_s_93	14741710	Biotin is the cofactor of pyruvate carboxylase (PC), which catalyzes pyruvate to oxaloacetate,  and acetyl CoA carboxylase (ACC), which catalyzes acetyl CoA to malonyl CoA.	transcription
53830	7	334917	6	NULL	NULL	0	NULL	biotin			is cofactor of					ACC					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_314_3_824_s_93	14741710	Biotin is the cofactor of pyruvate carboxylase (PC), which catalyzes pyruvate to oxaloacetate,  and acetyl CoA carboxylase (ACC), which catalyzes acetyl CoA to malonyl CoA.	transcription
52149	1	334918	5	NULL	NULL	0	NULL	pyruvate	NULL		is carboxylated to	NULL				oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevnutr_22_0_221_s_92	12055344	Pyruvate  carboxylase catalyzes the carboxylation of pyruvate to generate oxaloacetate and  therefore serves as an anapleurotic reaction that replenishes citric acid cycle intermediates  and catalyzes a required step in gluconeogenesis.	transcription
52150	2	334918	5	NULL	NULL	0	NULL	pyruvate carboxylase	NULL		catalyzes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevnutr_22_0_221_s_92	12055344	Pyruvate  carboxylase catalyzes the carboxylation of pyruvate to generate oxaloacetate and  therefore serves as an anapleurotic reaction that replenishes citric acid cycle intermediates  and catalyzes a required step in gluconeogenesis.	transcription
52151	3	334918	5	NULL	NULL	0	NULL	statement 1	NULL		is a type of	NULL				anapleurotic reaction	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevnutr_22_0_221_s_92	12055344	Pyruvate  carboxylase catalyzes the carboxylation of pyruvate to generate oxaloacetate and  therefore serves as an anapleurotic reaction that replenishes citric acid cycle intermediates  and catalyzes a required step in gluconeogenesis.	transcription
52152	4	334918	5	NULL	NULL	0	NULL	statement 1	NULL		replenishes	NULL				citric acid cycle intermediates	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevnutr_22_0_221_s_92	12055344	Pyruvate  carboxylase catalyzes the carboxylation of pyruvate to generate oxaloacetate and  therefore serves as an anapleurotic reaction that replenishes citric acid cycle intermediates  and catalyzes a required step in gluconeogenesis.	transcription
52153	5	334918	5	NULL	NULL	0	NULL	statement 1	NULL		catalyzes	NULL				gluconeogenesis	NULL	required step in			NULL		0	NULL	NULL	NULL	gw70_annurevnutr_22_0_221_s_92	12055344	Pyruvate  carboxylase catalyzes the carboxylation of pyruvate to generate oxaloacetate and  therefore serves as an anapleurotic reaction that replenishes citric acid cycle intermediates  and catalyzes a required step in gluconeogenesis.	transcription
53831	1	334918	6	NULL	NULL	0	NULL	pyruvate			is carboxylated to					oxaloacetate					NULL		0	NULL	NULL	NULL	gw70_annurevnutr_22_0_221_s_92	12055344	Pyruvate  carboxylase catalyzes the carboxylation of pyruvate to generate oxaloacetate and  therefore serves as an anapleurotic reaction that replenishes citric acid cycle intermediates  and catalyzes a required step in gluconeogenesis.	transcription
53832	2	334918	6	NULL	NULL	0	NULL	Pyruvate carboxylase			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw70_annurevnutr_22_0_221_s_92	12055344	Pyruvate  carboxylase catalyzes the carboxylation of pyruvate to generate oxaloacetate and  therefore serves as an anapleurotic reaction that replenishes citric acid cycle intermediates  and catalyzes a required step in gluconeogenesis.	transcription
53833	3	334918	6	NULL	NULL	0	NULL	Pyruvate carboxylase			serves as an					anapleurotic reaction					NULL		0	NULL	NULL	NULL	gw70_annurevnutr_22_0_221_s_92	12055344	Pyruvate  carboxylase catalyzes the carboxylation of pyruvate to generate oxaloacetate and  therefore serves as an anapleurotic reaction that replenishes citric acid cycle intermediates  and catalyzes a required step in gluconeogenesis.	transcription
53834	4	334918	6	NULL	NULL	0	NULL	Pyruvate carboxylase			replenishes					citric acid cycle intermediates					NULL		0	NULL	NULL	NULL	gw70_annurevnutr_22_0_221_s_92	12055344	Pyruvate  carboxylase catalyzes the carboxylation of pyruvate to generate oxaloacetate and  therefore serves as an anapleurotic reaction that replenishes citric acid cycle intermediates  and catalyzes a required step in gluconeogenesis.	transcription
52154	1	334919	5	NULL	NULL	0	NULL	PC	NULL		is important for	NULL				gluconeogenic pathway	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_23_18_3621_s_17	15329673	As the first enzyme in the gluconeogenic pathway, PC catalyzes  the ATP-driven conversion of pyruvate to oxaloacetate using HCO3- and Mg2+ (  et al).	transcription
52155	2	334919	5	NULL	NULL	0	NULL	pyruvate	NULL		is converted to	NULL				oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_23_18_3621_s_17	15329673	As the first enzyme in the gluconeogenic pathway, PC catalyzes  the ATP-driven conversion of pyruvate to oxaloacetate using HCO3- and Mg2+ (  et al).	transcription
52156	3	334919	5	NULL	NULL	0	NULL	statement 1	NULL		is driven by	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_23_18_3621_s_17	15329673	As the first enzyme in the gluconeogenic pathway, PC catalyzes  the ATP-driven conversion of pyruvate to oxaloacetate using HCO3- and Mg2+ (  et al).	transcription
52157	4	334919	5	NULL	NULL	0	NULL	PC	NULL		catalyzes	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_23_18_3621_s_17	15329673	As the first enzyme in the gluconeogenic pathway, PC catalyzes  the ATP-driven conversion of pyruvate to oxaloacetate using HCO3- and Mg2+ (  et al).	transcription
52158	5	334919	5	NULL	NULL	0	NULL	HCO3-	NULL		is required for	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_23_18_3621_s_17	15329673	As the first enzyme in the gluconeogenic pathway, PC catalyzes  the ATP-driven conversion of pyruvate to oxaloacetate using HCO3- and Mg2+ (  et al).	transcription
52159	6	334919	5	NULL	NULL	0	NULL	Mg2+	NULL		is required for	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_embo_23_18_3621_s_17	15329673	As the first enzyme in the gluconeogenic pathway, PC catalyzes  the ATP-driven conversion of pyruvate to oxaloacetate using HCO3- and Mg2+ (  et al).	transcription
53835	1	334919	6	NULL	NULL	0	NULL	pyruvate			is converted to					oxaloacetate					NULL		0	NULL	NULL	NULL	gw70_embo_23_18_3621_s_17	15329673	As the first enzyme in the gluconeogenic pathway, PC catalyzes  the ATP-driven conversion of pyruvate to oxaloacetate using HCO3- and Mg2+ (  et al).	transcription
53836	2	334919	6	NULL	NULL	0	NULL	statement 1			is dependent on					ATP					NULL		0	NULL	NULL	NULL	gw70_embo_23_18_3621_s_17	15329673	As the first enzyme in the gluconeogenic pathway, PC catalyzes  the ATP-driven conversion of pyruvate to oxaloacetate using HCO3- and Mg2+ (  et al).	transcription
53837	3	334919	6	NULL	NULL	0	NULL	PC			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw70_embo_23_18_3621_s_17	15329673	As the first enzyme in the gluconeogenic pathway, PC catalyzes  the ATP-driven conversion of pyruvate to oxaloacetate using HCO3- and Mg2+ (  et al).	transcription
53838	4	334919	6	NULL	NULL	0	NULL	PC			is 					enzyme in the gluconeogenic pathway		first			NULL		0	NULL	NULL	NULL	gw70_embo_23_18_3621_s_17	15329673	As the first enzyme in the gluconeogenic pathway, PC catalyzes  the ATP-driven conversion of pyruvate to oxaloacetate using HCO3- and Mg2+ (  et al).	transcription
53839	5	334919	6	NULL	NULL	0	NULL	statement 3			uses					HCO3-					NULL		0	NULL	NULL	NULL	gw70_embo_23_18_3621_s_17	15329673	As the first enzyme in the gluconeogenic pathway, PC catalyzes  the ATP-driven conversion of pyruvate to oxaloacetate using HCO3- and Mg2+ (  et al).	transcription
53840	6	334919	6	NULL	NULL	0	NULL	statement 3			uses					Mg2+					NULL		0	NULL	NULL	NULL	gw70_embo_23_18_3621_s_17	15329673	As the first enzyme in the gluconeogenic pathway, PC catalyzes  the ATP-driven conversion of pyruvate to oxaloacetate using HCO3- and Mg2+ (  et al).	transcription
52160	1	334920	5	NULL	NULL	0	NULL		NULL	luciferase activity of	is induced by	NULL			HRE	pyruvate	NULL				NULL	U251-HRE cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_144	16223732	Cysteine and histidine also lowered HRE-luciferase activity induced by pyruvate or oxaloacetate in the U251-HRE cells ( Fig. 2 D).	transcription
52161	2	334920	5	NULL	NULL	0	NULL		NULL	luciferase activity of	is induced by	NULL			HRE	oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_144	16223732	Cysteine and histidine also lowered HRE-luciferase activity induced by pyruvate or oxaloacetate in the U251-HRE cells ( Fig. 2 D).	transcription
52162	3	334920	5	NULL	NULL	0	NULL	cysteine	NULL		lowers	NULL				statement 1	NULL				NULL	U251-HRE cells	0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_144	16223732	Cysteine and histidine also lowered HRE-luciferase activity induced by pyruvate or oxaloacetate in the U251-HRE cells ( Fig. 2 D).	transcription
52163	4	334920	5	NULL	NULL	0	NULL	cysteine	NULL		lowers	NULL				statement 2	NULL				NULL	U251-HRE cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_144	16223732	Cysteine and histidine also lowered HRE-luciferase activity induced by pyruvate or oxaloacetate in the U251-HRE cells ( Fig. 2 D).	transcription
52164	5	334920	5	NULL	NULL	0	NULL	histidine	NULL		lowers	NULL				statement 1	NULL				NULL	U251-HRE cells	0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_144	16223732	Cysteine and histidine also lowered HRE-luciferase activity induced by pyruvate or oxaloacetate in the U251-HRE cells ( Fig. 2 D).	transcription
52165	6	334920	5	NULL	NULL	0	NULL	histidine	NULL		lowers	NULL				statement 2	NULL				NULL	U251-HRE cells	0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_144	16223732	Cysteine and histidine also lowered HRE-luciferase activity induced by pyruvate or oxaloacetate in the U251-HRE cells ( Fig. 2 D).	transcription
52166	7	334920	5	NULL	NULL	0	NULL	statement 1	NULL		is an alternative to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_144	16223732	Cysteine and histidine also lowered HRE-luciferase activity induced by pyruvate or oxaloacetate in the U251-HRE cells ( Fig. 2 D).	transcription
53841	1	334920	6	NULL	NULL	0	NULL	pyruvate			induces					HRE-luciferase		activity of			NULL	U251-HRE cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_144	16223732	Cysteine and histidine also lowered HRE-luciferase activity induced by pyruvate or oxaloacetate in the U251-HRE cells ( Fig. 2 D).	transcription
53842	2	334920	6	NULL	NULL	0	NULL	oxaloacetate			induces					HRE-luciferase		activity of			NULL	U251-HRE cells	0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_144	16223732	Cysteine and histidine also lowered HRE-luciferase activity induced by pyruvate or oxaloacetate in the U251-HRE cells ( Fig. 2 D).	transcription
53843	3	334920	6	NULL	NULL	0	NULL	cysteine			lowers					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_144	16223732	Cysteine and histidine also lowered HRE-luciferase activity induced by pyruvate or oxaloacetate in the U251-HRE cells ( Fig. 2 D).	transcription
53844	4	334920	6	NULL	NULL	0	NULL	cysteine			lowers					statement 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_144	16223732	Cysteine and histidine also lowered HRE-luciferase activity induced by pyruvate or oxaloacetate in the U251-HRE cells ( Fig. 2 D).	transcription
53845	5	334920	6	NULL	NULL	0	NULL	histidine			lowers					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_144	16223732	Cysteine and histidine also lowered HRE-luciferase activity induced by pyruvate or oxaloacetate in the U251-HRE cells ( Fig. 2 D).	transcription
53846	6	334920	6	NULL	NULL	0	NULL	histidine			lowers					statement 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_144	16223732	Cysteine and histidine also lowered HRE-luciferase activity induced by pyruvate or oxaloacetate in the U251-HRE cells ( Fig. 2 D).	transcription
52167	1	334921	5	NULL	NULL	0	NULL	HIF-1alpha	NULL		is induced by	NULL				pyruvate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_159	16223732	HIF-1alpha induced by pyruvate, oxaloacetate, or the HPH inhibitor DMOG did not contain hydroxyproline ( Fig. 3 D).	transcription
52168	2	334921	5	NULL	NULL	0	NULL	HIF-1alpha	NULL		is induced by	NULL				oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_159	16223732	HIF-1alpha induced by pyruvate, oxaloacetate, or the HPH inhibitor DMOG did not contain hydroxyproline ( Fig. 3 D).	transcription
52169	3	334921	5	NULL	NULL	0	NULL	HIF-1alpha	NULL		is induced by	NULL				DMOG	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_159	16223732	HIF-1alpha induced by pyruvate, oxaloacetate, or the HPH inhibitor DMOG did not contain hydroxyproline ( Fig. 3 D).	transcription
52170	4	334921	5	NULL	NULL	0	NULL	DMOG	NULL		is an inhibitor of	NULL				HPH	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_159	16223732	HIF-1alpha induced by pyruvate, oxaloacetate, or the HPH inhibitor DMOG did not contain hydroxyproline ( Fig. 3 D).	transcription
52171	5	334921	5	NULL	NULL	0	NULL	HIF-1alpha	NULL		does not contain	NULL					NULL		hydroxyproline		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_159	16223732	HIF-1alpha induced by pyruvate, oxaloacetate, or the HPH inhibitor DMOG did not contain hydroxyproline ( Fig. 3 D).	transcription
53847	1	334921	6	NULL	NULL	0	NULL	pyruvate			induces					HIF-1alpha					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_159	16223732	HIF-1alpha induced by pyruvate, oxaloacetate, or the HPH inhibitor DMOG did not contain hydroxyproline ( Fig. 3 D).	transcription
53848	2	334921	6	NULL	NULL	0	NULL	oxaloacetate			induces					HIF-1alpha					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_159	16223732	HIF-1alpha induced by pyruvate, oxaloacetate, or the HPH inhibitor DMOG did not contain hydroxyproline ( Fig. 3 D).	transcription
53849	3	334921	6	NULL	NULL	0	NULL	DMOG			induces					HIF-1alpha					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_159	16223732	HIF-1alpha induced by pyruvate, oxaloacetate, or the HPH inhibitor DMOG did not contain hydroxyproline ( Fig. 3 D).	transcription
53850	4	334921	6	NULL	NULL	0	NULL	DMOG			is a type of					HPH inhibitor					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_159	16223732	HIF-1alpha induced by pyruvate, oxaloacetate, or the HPH inhibitor DMOG did not contain hydroxyproline ( Fig. 3 D).	transcription
53851	5	334921	6	NULL	NULL	0	NULL	HIF-1alpha			does not contain					hydroxyproline					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_159	16223732	HIF-1alpha induced by pyruvate, oxaloacetate, or the HPH inhibitor DMOG did not contain hydroxyproline ( Fig. 3 D).	transcription
52172	1	334922	5	NULL	NULL	0	NULL	pyruvate	NULL		induce	NULL				HIF-1alpha	NULL	accumulation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_241	16223732	The ascorbate reversibility of pyruvate- and oxaloacetate-induced HIF-1alpha accumulation thus suggested that these 2-oxoacids could somehow inactivate cellular HPHs.	transcription
52173	2	334922	5	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				ascorbate reversibility	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_241	16223732	The ascorbate reversibility of pyruvate- and oxaloacetate-induced HIF-1alpha accumulation thus suggested that these 2-oxoacids could somehow inactivate cellular HPHs.	transcription
52174	3	334922	5	NULL	NULL	0	NULL	oxaloacetate	NULL		induce	NULL				HIF-1alpha	NULL	accumulation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_241	16223732	The ascorbate reversibility of pyruvate- and oxaloacetate-induced HIF-1alpha accumulation thus suggested that these 2-oxoacids could somehow inactivate cellular HPHs.	transcription
52175	4	334922	5	NULL	NULL	0	NULL	statement 3	NULL		leads to	NULL				ascorbate reversibility	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_241	16223732	The ascorbate reversibility of pyruvate- and oxaloacetate-induced HIF-1alpha accumulation thus suggested that these 2-oxoacids could somehow inactivate cellular HPHs.	transcription
52176	5	334922	5	NULL	NULL	0	NULL	pyruvate	NULL		is a type of	NULL				2-oxoacids	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_241	16223732	The ascorbate reversibility of pyruvate- and oxaloacetate-induced HIF-1alpha accumulation thus suggested that these 2-oxoacids could somehow inactivate cellular HPHs.	transcription
52177	6	334922	5	NULL	NULL	0	NULL	oxaloacetate	NULL		is a type of	NULL				2-oxoacids	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_241	16223732	The ascorbate reversibility of pyruvate- and oxaloacetate-induced HIF-1alpha accumulation thus suggested that these 2-oxoacids could somehow inactivate cellular HPHs.	transcription
52178	7	334922	5	NULL	NULL	0	NULL	pyruvate	NULL		inactivates	NULL				HPHs	NULL	cellular			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_241	16223732	The ascorbate reversibility of pyruvate- and oxaloacetate-induced HIF-1alpha accumulation thus suggested that these 2-oxoacids could somehow inactivate cellular HPHs.	transcription
52179	8	334922	5	NULL	NULL	0	NULL	oxaloacetate	NULL		inactivates	NULL				HPHs	NULL	cellular			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_241	16223732	The ascorbate reversibility of pyruvate- and oxaloacetate-induced HIF-1alpha accumulation thus suggested that these 2-oxoacids could somehow inactivate cellular HPHs.	transcription
53852	1	334922	6	NULL	NULL	0	NULL	pyruvate			induces					HIF-1alpha		accumulation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_241	16223732	The ascorbate reversibility of pyruvate- and oxaloacetate-induced HIF-1alpha accumulation thus suggested that these 2-oxoacids could somehow inactivate cellular HPHs.	transcription
53853	2	334922	6	NULL	NULL	0	NULL	oxaloacetate			induces					HIF-1alpha		accumulation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_241	16223732	The ascorbate reversibility of pyruvate- and oxaloacetate-induced HIF-1alpha accumulation thus suggested that these 2-oxoacids could somehow inactivate cellular HPHs.	transcription
53854	3	334922	6	NULL	NULL	0	NULL	oxoacids			inactivate					HPH					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_241	16223732	The ascorbate reversibility of pyruvate- and oxaloacetate-induced HIF-1alpha accumulation thus suggested that these 2-oxoacids could somehow inactivate cellular HPHs.	transcription
52180	1	334924	5	NULL	NULL	0	NULL	pyruvate	NULL		induce	NULL				HIF-1alpha	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_271	16223732	The addition of Fe(II) to cultured cells also prevented HIF-1alpha induction by pyruvate and oxaloacetate.	transcription
52181	2	334924	5	NULL	NULL	0	NULL	oxaloacetate	NULL		induce	NULL				HIF-1alpha	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_271	16223732	The addition of Fe(II) to cultured cells also prevented HIF-1alpha induction by pyruvate and oxaloacetate.	transcription
52182	3	334924	5	NULL	NULL	0	NULL	Fe(II)	NULL	addition of	prevents	NULL				statement 1	NULL				NULL	cultured cells	0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_271	16223732	The addition of Fe(II) to cultured cells also prevented HIF-1alpha induction by pyruvate and oxaloacetate.	transcription
53855	1	334924	6	NULL	NULL	0	NULL	pyruvate			induces					HIF-1alpha		induction of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_271	16223732	The addition of Fe(II) to cultured cells also prevented HIF-1alpha induction by pyruvate and oxaloacetate.	transcription
53857	2	334924	6	NULL	NULL	0	NULL	oxaloacetate			induces					HIF-1alpha		induction of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_271	16223732	The addition of Fe(II) to cultured cells also prevented HIF-1alpha induction by pyruvate and oxaloacetate.	transcription
52483	1	334925	5	NULL	NULL	0	NULL	metabolic pathways	NULL		regulates	NULL				HPH	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_358	16223732	The origin of pyruvate, oxaloacetate, and the branched chain 2-oxoacids via diverse metabolic routes underscores the potential for HPH regulation by metabolic pathways.	transcription
52183	1	334926	5	NULL	NULL	0	NULL	oxaloacetate	NULL		is synthesized from	NULL				PEP	NULL				NULL	Escherichia coli	NULL	NULL	NULL	NULL	gw60_febslett_412_3_531_s_9	9276461	Escherichia coli synthesizes oxaloacetate not from pyruvate, but from phosphoenolpyruvate (PEP) in a reaction catalyzed by PEP carboxylase [ 2,   5].	transcription
52184	2	334926	5	NULL	NULL	0	NULL	PEP carboxylase	NULL		catalyzes	NULL				statement 1	NULL				NULL	Escherichia coli	0	NULL	NULL	NULL	gw60_febslett_412_3_531_s_9	9276461	Escherichia coli synthesizes oxaloacetate not from pyruvate, but from phosphoenolpyruvate (PEP) in a reaction catalyzed by PEP carboxylase [ 2,   5].	transcription
52185	3	334926	5	NULL	NULL	0	NULL	PEP	NULL		is	NULL				phosphoenolpyruvate	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_412_3_531_s_9	9276461	Escherichia coli synthesizes oxaloacetate not from pyruvate, but from phosphoenolpyruvate (PEP) in a reaction catalyzed by PEP carboxylase [ 2,   5].	transcription
53858	1	334926	6	NULL	NULL	0	NULL	oxaloacetate			is synthesized from					PEP					NULL	Escherichia coli	NULL	NULL	NULL	NULL	gw60_febslett_412_3_531_s_9	9276461	Escherichia coli synthesizes oxaloacetate not from pyruvate, but from phosphoenolpyruvate (PEP) in a reaction catalyzed by PEP carboxylase [ 2,   5].	transcription
53859	2	334926	6	NULL	NULL	0	NULL	PEP			is					phosphoenolpyruvate					NULL		0	NULL	NULL	NULL	gw60_febslett_412_3_531_s_9	9276461	Escherichia coli synthesizes oxaloacetate not from pyruvate, but from phosphoenolpyruvate (PEP) in a reaction catalyzed by PEP carboxylase [ 2,   5].	transcription
53860	3	334926	6	NULL	NULL	0	NULL	PEP carboxylase			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw60_febslett_412_3_531_s_9	9276461	Escherichia coli synthesizes oxaloacetate not from pyruvate, but from phosphoenolpyruvate (PEP) in a reaction catalyzed by PEP carboxylase [ 2,   5].	transcription
52186	1	334927	5	NULL	NULL	0	NULL	Pyc	NULL		is a type of	NULL				biotin-containing enzyme	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_66_3_1223_s_12	10698798	Pyc is a biotin-containing enzyme that catalyzes the ATP-dependent carboxylation of pyruvate to form oxaloacetate (OAA) ( 4).	transcription
52187	2	334927	5	NULL	NULL	0	NULL	pyruvate	NULL		is carboxylated to	NULL				oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_66_3_1223_s_12	10698798	Pyc is a biotin-containing enzyme that catalyzes the ATP-dependent carboxylation of pyruvate to form oxaloacetate (OAA) ( 4).	transcription
52188	3	334927	5	NULL	NULL	0	NULL	statement 2	NULL		is dependent on	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_66_3_1223_s_12	10698798	Pyc is a biotin-containing enzyme that catalyzes the ATP-dependent carboxylation of pyruvate to form oxaloacetate (OAA) ( 4).	transcription
52189	4	334927	5	NULL	NULL	0	NULL	Pyc	NULL		catalyzes	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_66_3_1223_s_12	10698798	Pyc is a biotin-containing enzyme that catalyzes the ATP-dependent carboxylation of pyruvate to form oxaloacetate (OAA) ( 4).	transcription
52190	5	334927	5	NULL	NULL	0	NULL	oxaloacetate	NULL		is	NULL				OAA	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_66_3_1223_s_12	10698798	Pyc is a biotin-containing enzyme that catalyzes the ATP-dependent carboxylation of pyruvate to form oxaloacetate (OAA) ( 4).	transcription
53861	1	334927	6	NULL	NULL	0	NULL	pyruvate			is carboxylated to					oxaloacetate					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_66_3_1223_s_12	10698798	Pyc is a biotin-containing enzyme that catalyzes the ATP-dependent carboxylation of pyruvate to form oxaloacetate (OAA) ( 4).	transcription
53862	2	334927	6	NULL	NULL	0	NULL	OAA			is					oxaloacetate					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_66_3_1223_s_12	10698798	Pyc is a biotin-containing enzyme that catalyzes the ATP-dependent carboxylation of pyruvate to form oxaloacetate (OAA) ( 4).	transcription
53863	3	334927	6	NULL	NULL	0	NULL	statement 1			is dependent on					ATP					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_66_3_1223_s_12	10698798	Pyc is a biotin-containing enzyme that catalyzes the ATP-dependent carboxylation of pyruvate to form oxaloacetate (OAA) ( 4).	transcription
53864	4	334927	6	NULL	NULL	0	NULL	Pyc			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_66_3_1223_s_12	10698798	Pyc is a biotin-containing enzyme that catalyzes the ATP-dependent carboxylation of pyruvate to form oxaloacetate (OAA) ( 4).	transcription
53865	5	334927	6	NULL	NULL	0	NULL	Pyc			is					biotin-containing enzyme family					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_66_3_1223_s_12	10698798	Pyc is a biotin-containing enzyme that catalyzes the ATP-dependent carboxylation of pyruvate to form oxaloacetate (OAA) ( 4).	transcription
52191	1	334929	5	NULL	NULL	0	NULL	succinate dehydrogenase	NULL		is inhibited by	NULL				oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_40_25019_s_170	8798784	Such an interaction has been suggested to be responsible for the inhibition of succinate dehydrogenase by oxaloacetate ( 37), which, like pyruvate, is an alpha-keto acid.	transcription
52192	2	334929	5	NULL	NULL	0	NULL	oxaloacetate	NULL		is a type of	NULL				alpha-keto acid	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_40_25019_s_170	8798784	Such an interaction has been suggested to be responsible for the inhibition of succinate dehydrogenase by oxaloacetate ( 37), which, like pyruvate, is an alpha-keto acid.	transcription
52193	3	334929	5	NULL	NULL	0	NULL	pyruvate	NULL		is a type of	NULL				alpha-keto acid	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_40_25019_s_170	8798784	Such an interaction has been suggested to be responsible for the inhibition of succinate dehydrogenase by oxaloacetate ( 37), which, like pyruvate, is an alpha-keto acid.	transcription
54320	1	334929	6	NULL	NULL	0	NULL	oxaloacetate			inhibits					succinate dehydrogenase					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_40_25019_s_170	8798784	Such an interaction has been suggested to be responsible for the inhibition of succinate dehydrogenase by oxaloacetate ( 37), which, like pyruvate, is an alpha-keto acid.	transcription
54330	2	334929	6	NULL	NULL	0	NULL	succinate dehydrogenase			is a type of					alpha-keto acid					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_40_25019_s_170	8798784	Such an interaction has been suggested to be responsible for the inhibition of succinate dehydrogenase by oxaloacetate ( 37), which, like pyruvate, is an alpha-keto acid.	transcription
52194	1	334930	5	NULL	NULL	0	NULL	Oxalate	NULL		is a dead-end analogue of 	NULL				enolpyruvate	NULL				NULL		0	NULL	NULL	NULL	gw70_febslett_570_1_217_s_132	15251467	Oxalate (dead-end analogue of enolpyruvate) and malonate (dead-end analogue of oxaloacetate/pyruvate),  produced high inhibition on the activity ( Table 1).	transcription
52195	2	334930	5	NULL	NULL	0	NULL	malonate	NULL		is a dead-end analogue of	NULL				oxaloacetate/pyruvate	NULL				NULL		0	NULL	NULL	NULL	gw70_febslett_570_1_217_s_132	15251467	Oxalate (dead-end analogue of enolpyruvate) and malonate (dead-end analogue of oxaloacetate/pyruvate),  produced high inhibition on the activity ( Table 1).	transcription
52196	1	334931	5	NULL	NULL	0	NULL		NULL	absence of	allows	NULL	may	C5 carboxyl group		pyruvate	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_334	16223732	It is possible that the absence of a C5 carboxyl group allows pyruvate and oxaloacetate binding to interfere with allosteric enzyme mechanisms for the scheduled sequential binding of other reactants.	transcription
52197	2	334931	5	NULL	NULL	0	NULL		NULL	absence of	allows	NULL	may	C5 carboxyl group		oxaloacetate	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_334	16223732	It is possible that the absence of a C5 carboxyl group allows pyruvate and oxaloacetate binding to interfere with allosteric enzyme mechanisms for the scheduled sequential binding of other reactants.	transcription
52198	3	334931	5	NULL	NULL	0	NULL	statement 1	NULL		interfere with	NULL				allosteric enzyme	NULL	mechanism of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_334	16223732	It is possible that the absence of a C5 carboxyl group allows pyruvate and oxaloacetate binding to interfere with allosteric enzyme mechanisms for the scheduled sequential binding of other reactants.	transcription
52199	4	334931	5	NULL	NULL	0	NULL	statement 2	NULL		interfere with	NULL				allosteric enzyme	NULL	mechanism of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_334	16223732	It is possible that the absence of a C5 carboxyl group allows pyruvate and oxaloacetate binding to interfere with allosteric enzyme mechanisms for the scheduled sequential binding of other reactants.	transcription
52200	5	334931	5	NULL	NULL	0	NULL	statement 3	NULL		leads to	NULL				reactants	NULL	scheduled;;sequential binding of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_334	16223732	It is possible that the absence of a C5 carboxyl group allows pyruvate and oxaloacetate binding to interfere with allosteric enzyme mechanisms for the scheduled sequential binding of other reactants.	transcription
52201	6	334931	5	NULL	NULL	0	NULL	statement 4	NULL		leads to	NULL				reactants	NULL	scheduled;;sequential binding of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_334	16223732	It is possible that the absence of a C5 carboxyl group allows pyruvate and oxaloacetate binding to interfere with allosteric enzyme mechanisms for the scheduled sequential binding of other reactants.	transcription
52202	1	334932	5	NULL	NULL	0	NULL	acetyl-CoA	NULL		is carboxylated to	NULL				malonyl-CoA	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_19_13513_s_20	16533810	Acc1p catalyzes the first step of fatty acid biosynthesis ( i.e. the carboxylation of acetyl-CoA to malonyl-CoA), and Pyc1p and Pyc2p generate oxaloacetate from pyruvate.	transcription
52203	2	334932	5	NULL	NULL	0	NULL	statement 1	NULL		is first step of	NULL				fatty acid	NULL	biosynthesis of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_19_13513_s_20	16533810	Acc1p catalyzes the first step of fatty acid biosynthesis ( i.e. the carboxylation of acetyl-CoA to malonyl-CoA), and Pyc1p and Pyc2p generate oxaloacetate from pyruvate.	transcription
52204	3	334932	5	NULL	NULL	0	NULL	Acc1p	NULL		catalyzes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_19_13513_s_20	16533810	Acc1p catalyzes the first step of fatty acid biosynthesis ( i.e. the carboxylation of acetyl-CoA to malonyl-CoA), and Pyc1p and Pyc2p generate oxaloacetate from pyruvate.	transcription
52205	4	334932	5	NULL	NULL	0	NULL	oxaloacetate	NULL		is generated from	NULL				pyruvate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_19_13513_s_20	16533810	Acc1p catalyzes the first step of fatty acid biosynthesis ( i.e. the carboxylation of acetyl-CoA to malonyl-CoA), and Pyc1p and Pyc2p generate oxaloacetate from pyruvate.	transcription
52206	5	334932	5	NULL	NULL	0	NULL	Pyc1p	NULL		catalyzes	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_19_13513_s_20	16533810	Acc1p catalyzes the first step of fatty acid biosynthesis ( i.e. the carboxylation of acetyl-CoA to malonyl-CoA), and Pyc1p and Pyc2p generate oxaloacetate from pyruvate.	transcription
52207	6	334932	5	NULL	NULL	0	NULL	Pyc2p	NULL		catalyzes	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_19_13513_s_20	16533810	Acc1p catalyzes the first step of fatty acid biosynthesis ( i.e. the carboxylation of acetyl-CoA to malonyl-CoA), and Pyc1p and Pyc2p generate oxaloacetate from pyruvate.	transcription
54331	1	334932	6	NULL	NULL	0	NULL	acetyl-CoA			is carboxylated to					malonyl-CoA					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_19_13513_s_20	16533810	Acc1p catalyzes the first step of fatty acid biosynthesis ( i.e. the carboxylation of acetyl-CoA to malonyl-CoA), and Pyc1p and Pyc2p generate oxaloacetate from pyruvate.	transcription
54332	2	334932	6	NULL	NULL	0	NULL	Acc1p			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_19_13513_s_20	16533810	Acc1p catalyzes the first step of fatty acid biosynthesis ( i.e. the carboxylation of acetyl-CoA to malonyl-CoA), and Pyc1p and Pyc2p generate oxaloacetate from pyruvate.	transcription
54333	3	334932	6	NULL	NULL	0	NULL	oxaloacetate			is generated from					pyruvate					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_19_13513_s_20	16533810	Acc1p catalyzes the first step of fatty acid biosynthesis ( i.e. the carboxylation of acetyl-CoA to malonyl-CoA), and Pyc1p and Pyc2p generate oxaloacetate from pyruvate.	transcription
54334	4	334932	6	NULL	NULL	0	NULL	Pyc1p			plays a role in					statement 3					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_19_13513_s_20	16533810	Acc1p catalyzes the first step of fatty acid biosynthesis ( i.e. the carboxylation of acetyl-CoA to malonyl-CoA), and Pyc1p and Pyc2p generate oxaloacetate from pyruvate.	transcription
54335	5	334932	6	NULL	NULL	0	NULL	Pyc2p			plays a role in					statement 3					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_19_13513_s_20	16533810	Acc1p catalyzes the first step of fatty acid biosynthesis ( i.e. the carboxylation of acetyl-CoA to malonyl-CoA), and Pyc1p and Pyc2p generate oxaloacetate from pyruvate.	transcription
52208	1	334933	5	NULL	NULL	0	NULL	biotin	NULL	uptake of	is increased by	NULL				amino acid	NULL	starvation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_18_12381_s_347	16531611	Contrary to earlier speculations ( ), we propose that biotin uptake is increased by amino acid starvation to increase the activity of the biotin-dependent pyruvate carboxylases that generate oxaloacetate.	transcription
52209	2	334933	5	NULL	NULL	0	NULL	pyruvate carboxylases	NULL		generate	NULL				oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_18_12381_s_347	16531611	Contrary to earlier speculations ( ), we propose that biotin uptake is increased by amino acid starvation to increase the activity of the biotin-dependent pyruvate carboxylases that generate oxaloacetate.	transcription
52210	3	334933	5	NULL	NULL	0	NULL	statement 2	NULL		is dependent on	NULL				biotin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_18_12381_s_347	16531611	Contrary to earlier speculations ( ), we propose that biotin uptake is increased by amino acid starvation to increase the activity of the biotin-dependent pyruvate carboxylases that generate oxaloacetate.	transcription
52211	4	334933	5	NULL	NULL	0	NULL	statement 1	NULL		increases	NULL				pyruvate carboxylases	NULL	activity of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_18_12381_s_347	16531611	Contrary to earlier speculations ( ), we propose that biotin uptake is increased by amino acid starvation to increase the activity of the biotin-dependent pyruvate carboxylases that generate oxaloacetate.	transcription
54337	1	334933	6	NULL	NULL	0	NULL	biotin		uptake of	is increased by					amino acid starvation					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_18_12381_s_347	16531611	Contrary to earlier speculations ( ), we propose that biotin uptake is increased by amino acid starvation to increase the activity of the biotin-dependent pyruvate carboxylases that generate oxaloacetate.	transcription
54339	2	334933	6	NULL	NULL	0	NULL	pyruvate carboxylase			generates					oxaloacetate					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_18_12381_s_347	16531611	Contrary to earlier speculations ( ), we propose that biotin uptake is increased by amino acid starvation to increase the activity of the biotin-dependent pyruvate carboxylases that generate oxaloacetate.	transcription
54340	3	334933	6	NULL	NULL	0	NULL	statement 1			increases					pyruvate carboxylase		activity of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_18_12381_s_347	16531611	Contrary to earlier speculations ( ), we propose that biotin uptake is increased by amino acid starvation to increase the activity of the biotin-dependent pyruvate carboxylases that generate oxaloacetate.	transcription
52212	1	334934	5	NULL	NULL	0	NULL	PEPCK	NULL		is	NULL				phosphoenolpyruvate carboxykinase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_50_31475_s_15	9395482	In the liver, phosphoenolpyruvate carboxykinase (PEPCK) catalyzes the conversion of oxaloacetate to phosphoenolpyruvate and is considered the major rate-controlling enzyme in the pathway of gluconeogenesis from pyruvate, lactate, and alanine ( 8).	transcription
52213	2	334934	5	NULL	NULL	0	NULL	oxaloacetate	NULL		is converted to	NULL				phosphoenolpyruvate	NULL				NULL	liver	0	NULL	NULL	NULL	gw60_jbiolchem_272_50_31475_s_15	9395482	In the liver, phosphoenolpyruvate carboxykinase (PEPCK) catalyzes the conversion of oxaloacetate to phosphoenolpyruvate and is considered the major rate-controlling enzyme in the pathway of gluconeogenesis from pyruvate, lactate, and alanine ( 8).	transcription
52214	3	334934	5	NULL	NULL	0	NULL	PEPCK	NULL		catalyzes	NULL				statement 2	NULL				NULL	liver	0	NULL	NULL	NULL	gw60_jbiolchem_272_50_31475_s_15	9395482	In the liver, phosphoenolpyruvate carboxykinase (PEPCK) catalyzes the conversion of oxaloacetate to phosphoenolpyruvate and is considered the major rate-controlling enzyme in the pathway of gluconeogenesis from pyruvate, lactate, and alanine ( 8).	transcription
54342	1	334934	6	NULL	NULL	0	NULL	oxaloacetate			is converted to					phosphoenolpyruvate					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_50_31475_s_15	9395482	In the liver, phosphoenolpyruvate carboxykinase (PEPCK) catalyzes the conversion of oxaloacetate to phosphoenolpyruvate and is considered the major rate-controlling enzyme in the pathway of gluconeogenesis from pyruvate, lactate, and alanine ( 8).	transcription
54343	2	334934	6	NULL	NULL	0	NULL	PEPCK			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_50_31475_s_15	9395482	In the liver, phosphoenolpyruvate carboxykinase (PEPCK) catalyzes the conversion of oxaloacetate to phosphoenolpyruvate and is considered the major rate-controlling enzyme in the pathway of gluconeogenesis from pyruvate, lactate, and alanine ( 8).	transcription
52215	1	334935	5	NULL	NULL	0	NULL	pyruvate	NULL		inhibit	NULL	strongly			oxaloacetate	NULL	transamination of			NULL	brain homogenates	0	NULL	NULL	NULL	gw60_jneurosci_20_5_1809_s_192	10684882	Haslam and Krebs (1963)   found that 10 mM of pyruvate strongly inhibited oxaloacetate transamination in brain homogenates, and Dennis and Clark (1978)   observed the same in their nonsynaptic mitochondria.	transcription
52216	2	334935	5	NULL	NULL	0	NULL	pyruvate	NULL		inhibit	NULL	strongly			oxaloacetate	NULL	transamination of			NULL	nonsynaptic mitochondria	0	NULL	NULL	NULL	gw60_jneurosci_20_5_1809_s_192	10684882	Haslam and Krebs (1963)   found that 10 mM of pyruvate strongly inhibited oxaloacetate transamination in brain homogenates, and Dennis and Clark (1978)   observed the same in their nonsynaptic mitochondria.	transcription
54346	1	334935	6	NULL	NULL	0	NULL	pyruvate			inhibits		strongly			oxaloacetate		transamination of 			NULL	brain homogenates	NULL	NULL	NULL	NULL	gw60_jneurosci_20_5_1809_s_192	10684882	Haslam and Krebs (1963)   found that 10 mM of pyruvate strongly inhibited oxaloacetate transamination in brain homogenates, and Dennis and Clark (1978)   observed the same in their nonsynaptic mitochondria.	transcription
54347	2	334935	6	NULL	NULL	0	NULL	pyruvate			inhibits		strongly			oxaloacetate		transamination of 			NULL	nonsynaptic mitochondria	NULL	NULL	NULL	NULL	gw60_jneurosci_20_5_1809_s_192	10684882	Haslam and Krebs (1963)   found that 10 mM of pyruvate strongly inhibited oxaloacetate transamination in brain homogenates, and Dennis and Clark (1978)   observed the same in their nonsynaptic mitochondria.	transcription
52217	1	334937	5	NULL	NULL	0	NULL	oxaloacetate	NULL		is converted to	NULL				malate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_7470_s_160	14660628	An alternate metabolic pathway for oxaloacetate besides conversion to malate is citrate synthase-induced production of citrate and distal metabolism through malonyl-CoA or recycling to pyruvate through the pyruvate-citrate shuttle.	transcription
52218	2	334937	5	NULL	NULL	0	NULL	oxaloacetate	NULL		is converted to	NULL				citrate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_7470_s_160	14660628	An alternate metabolic pathway for oxaloacetate besides conversion to malate is citrate synthase-induced production of citrate and distal metabolism through malonyl-CoA or recycling to pyruvate through the pyruvate-citrate shuttle.	transcription
52219	3	334937	5	NULL	NULL	0	NULL	citrate synthase	NULL		catalyzes	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_7470_s_160	14660628	An alternate metabolic pathway for oxaloacetate besides conversion to malate is citrate synthase-induced production of citrate and distal metabolism through malonyl-CoA or recycling to pyruvate through the pyruvate-citrate shuttle.	transcription
52220	4	334937	5	NULL	NULL	0	NULL	oxaloacetate	NULL	distal metabolism of	occurs through	NULL				malonyl-CoA	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_7470_s_160	14660628	An alternate metabolic pathway for oxaloacetate besides conversion to malate is citrate synthase-induced production of citrate and distal metabolism through malonyl-CoA or recycling to pyruvate through the pyruvate-citrate shuttle.	transcription
52221	5	334937	5	NULL	NULL	0	NULL	oxaloacetate	NULL		is recycled to	NULL				pyruvate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_7470_s_160	14660628	An alternate metabolic pathway for oxaloacetate besides conversion to malate is citrate synthase-induced production of citrate and distal metabolism through malonyl-CoA or recycling to pyruvate through the pyruvate-citrate shuttle.	transcription
52222	6	334937	5	NULL	NULL	0	NULL	statement 5	NULL		occurs through	NULL				pyruvate-citrate shuttle	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_7470_s_160	14660628	An alternate metabolic pathway for oxaloacetate besides conversion to malate is citrate synthase-induced production of citrate and distal metabolism through malonyl-CoA or recycling to pyruvate through the pyruvate-citrate shuttle.	transcription
52223	7	334937	5	NULL	NULL	0	NULL	statement 4	NULL		is an alternative to	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_7470_s_160	14660628	An alternate metabolic pathway for oxaloacetate besides conversion to malate is citrate synthase-induced production of citrate and distal metabolism through malonyl-CoA or recycling to pyruvate through the pyruvate-citrate shuttle.	transcription
54352	1	334937	6	NULL	NULL	0	NULL	citrate synthase			induces					citrate		production of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_7470_s_160	14660628	An alternate metabolic pathway for oxaloacetate besides conversion to malate is citrate synthase-induced production of citrate and distal metabolism through malonyl-CoA or recycling to pyruvate through the pyruvate-citrate shuttle.	transcription
52224	1	334938	5	NULL	NULL	0	NULL	oxaloacetate	NULL		is synthesized from	NULL				pyruvate	NULL				NULL	S. cerevisiae	0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21044_s_23	10409655	In  S. cerevisiae, the anaplerotic synthesis of oxaloacetate from pyruvate is catalyzed by pyruvate carboxylase, an exclusively cytosolic enzyme, in contrast to many higher organisms in which this enzyme is mitochondrial ( 14,  18).	transcription
52225	2	334938	5	NULL	NULL	0	NULL	pyruvate carboxylase	NULL		catalyzes	NULL				statement 1	NULL				NULL	S. cerevisiae	0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21044_s_23	10409655	In  S. cerevisiae, the anaplerotic synthesis of oxaloacetate from pyruvate is catalyzed by pyruvate carboxylase, an exclusively cytosolic enzyme, in contrast to many higher organisms in which this enzyme is mitochondrial ( 14,  18).	transcription
52226	3	334938	5	NULL	NULL	0	NULL	statement 1	NULL		is a type of	NULL				anaplerotic reaction	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21044_s_23	10409655	In  S. cerevisiae, the anaplerotic synthesis of oxaloacetate from pyruvate is catalyzed by pyruvate carboxylase, an exclusively cytosolic enzyme, in contrast to many higher organisms in which this enzyme is mitochondrial ( 14,  18).	transcription
52227	4	334938	5	NULL	NULL	0	NULL	pyruvate carboxylase	NULL		is present in	NULL	exclusively			cytosol	NULL				NULL	S. cerevisiae	0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21044_s_23	10409655	In  S. cerevisiae, the anaplerotic synthesis of oxaloacetate from pyruvate is catalyzed by pyruvate carboxylase, an exclusively cytosolic enzyme, in contrast to many higher organisms in which this enzyme is mitochondrial ( 14,  18).	transcription
52228	5	334938	5	NULL	NULL	0	NULL	pyruvate carboxylase	NULL		is present in	NULL				mitochondria	NULL				NULL	higher organisms	0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21044_s_23	10409655	In  S. cerevisiae, the anaplerotic synthesis of oxaloacetate from pyruvate is catalyzed by pyruvate carboxylase, an exclusively cytosolic enzyme, in contrast to many higher organisms in which this enzyme is mitochondrial ( 14,  18).	transcription
54355	1	334938	6	NULL	NULL	0	NULL	oxaloacetate			is synthesized from					pyruvate					NULL	S. cerevisiae	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_30_21044_s_23	10409655	In  S. cerevisiae, the anaplerotic synthesis of oxaloacetate from pyruvate is catalyzed by pyruvate carboxylase, an exclusively cytosolic enzyme, in contrast to many higher organisms in which this enzyme is mitochondrial ( 14,  18).	transcription
54356	2	334938	6	NULL	NULL	0	NULL	statement 1			is catalyzed by					pyruvate carboxylase					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21044_s_23	10409655	In  S. cerevisiae, the anaplerotic synthesis of oxaloacetate from pyruvate is catalyzed by pyruvate carboxylase, an exclusively cytosolic enzyme, in contrast to many higher organisms in which this enzyme is mitochondrial ( 14,  18).	transcription
54357	3	334938	6	NULL	NULL	0	NULL	pyruvate carboxylase			is a type of					cytosolic enzyme					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21044_s_23	10409655	In  S. cerevisiae, the anaplerotic synthesis of oxaloacetate from pyruvate is catalyzed by pyruvate carboxylase, an exclusively cytosolic enzyme, in contrast to many higher organisms in which this enzyme is mitochondrial ( 14,  18).	transcription
52229	1	334939	5	NULL	NULL	0	NULL	mitochondria	NULL		oxidizes	NULL				pyruvate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21044_s_78	10409655	It is known that mitochondria do not oxidize pyruvate unless malate is added, since the oxaloacetate produced by malate dehydrogenase reacts with acetyl-CoA, a potent inhibitor of pyruvate dehydrogenase ( 6).	transcription
52230	2	334939	5	NULL	NULL	0	NULL	statement 1	NULL		in the presence of	NULL	only			malate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21044_s_78	10409655	It is known that mitochondria do not oxidize pyruvate unless malate is added, since the oxaloacetate produced by malate dehydrogenase reacts with acetyl-CoA, a potent inhibitor of pyruvate dehydrogenase ( 6).	transcription
52231	3	334939	5	NULL	NULL	0	NULL	oxaloacetate	NULL		is produced by	NULL				malate dehydrogenase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21044_s_78	10409655	It is known that mitochondria do not oxidize pyruvate unless malate is added, since the oxaloacetate produced by malate dehydrogenase reacts with acetyl-CoA, a potent inhibitor of pyruvate dehydrogenase ( 6).	transcription
52232	4	334939	5	NULL	NULL	0	NULL	statement 3	NULL		reacts with	NULL				acetyl-CoA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21044_s_78	10409655	It is known that mitochondria do not oxidize pyruvate unless malate is added, since the oxaloacetate produced by malate dehydrogenase reacts with acetyl-CoA, a potent inhibitor of pyruvate dehydrogenase ( 6).	transcription
52233	5	334939	5	NULL	NULL	0	NULL	acetyl-CoA	NULL		is an inhibitor of	NULL	potent			pyruvate dehydrogenase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21044_s_78	10409655	It is known that mitochondria do not oxidize pyruvate unless malate is added, since the oxaloacetate produced by malate dehydrogenase reacts with acetyl-CoA, a potent inhibitor of pyruvate dehydrogenase ( 6).	transcription
54358	1	334939	6	NULL	NULL	0	NULL	oxaloacetate			is produced by					malate dehydrogenase					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21044_s_78	10409655	It is known that mitochondria do not oxidize pyruvate unless malate is added, since the oxaloacetate produced by malate dehydrogenase reacts with acetyl-CoA, a potent inhibitor of pyruvate dehydrogenase ( 6).	transcription
54359	2	334939	6	NULL	NULL	0	NULL	oxaloacetate			reacts with					acetyl-CoA					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21044_s_78	10409655	It is known that mitochondria do not oxidize pyruvate unless malate is added, since the oxaloacetate produced by malate dehydrogenase reacts with acetyl-CoA, a potent inhibitor of pyruvate dehydrogenase ( 6).	transcription
54360	3	334939	6	NULL	NULL	0	NULL	acetyl-CoA			is an inhibitor of		potent			pyruvate dehydrogenase					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21044_s_78	10409655	It is known that mitochondria do not oxidize pyruvate unless malate is added, since the oxaloacetate produced by malate dehydrogenase reacts with acetyl-CoA, a potent inhibitor of pyruvate dehydrogenase ( 6).	transcription
54361	4	334939	6	NULL	NULL	0	NULL	mitochondria			do not oxidize					pyruvate					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21044_s_78	10409655	It is known that mitochondria do not oxidize pyruvate unless malate is added, since the oxaloacetate produced by malate dehydrogenase reacts with acetyl-CoA, a potent inhibitor of pyruvate dehydrogenase ( 6).	transcription
54362	5	334939	6	NULL	NULL	0	NULL	statement 4			occurs in presence of					malate					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21044_s_78	10409655	It is known that mitochondria do not oxidize pyruvate unless malate is added, since the oxaloacetate produced by malate dehydrogenase reacts with acetyl-CoA, a potent inhibitor of pyruvate dehydrogenase ( 6).	transcription
52234	1	334940	5	NULL	NULL	0	NULL	palmitate	NULL	oxidation of	results in	NULL				acetyl-CoA	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1757_1_57_s_240	16375848	Thus, an increase in acetyl-CoA content from palmitate oxidation leads up to inhibition  of pyruvate dehydrogenase activity, decreasing the conversion of pyruvate to acetyl-CoA,  but also enhances pyruvate carboxylase activity, raising the conversion of pyruvate  to oxaloacetate that entries into the Krebs cycle being then oxidized   [57].	transcription
52235	2	334940	5	NULL	NULL	0	NULL	acetyl-CoA	NULL		inhibits	NULL				pyruvate dehydrogenase	NULL	activity of			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1757_1_57_s_240	16375848	Thus, an increase in acetyl-CoA content from palmitate oxidation leads up to inhibition  of pyruvate dehydrogenase activity, decreasing the conversion of pyruvate to acetyl-CoA,  but also enhances pyruvate carboxylase activity, raising the conversion of pyruvate  to oxaloacetate that entries into the Krebs cycle being then oxidized   [57].	transcription
52236	3	334940	5	NULL	NULL	0	NULL	pyruvate	NULL		is converted to	NULL				acetyl-CoA	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1757_1_57_s_240	16375848	Thus, an increase in acetyl-CoA content from palmitate oxidation leads up to inhibition  of pyruvate dehydrogenase activity, decreasing the conversion of pyruvate to acetyl-CoA,  but also enhances pyruvate carboxylase activity, raising the conversion of pyruvate  to oxaloacetate that entries into the Krebs cycle being then oxidized   [57].	transcription
52237	4	334940	5	NULL	NULL	0	NULL	statement 2	NULL		decreases	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1757_1_57_s_240	16375848	Thus, an increase in acetyl-CoA content from palmitate oxidation leads up to inhibition  of pyruvate dehydrogenase activity, decreasing the conversion of pyruvate to acetyl-CoA,  but also enhances pyruvate carboxylase activity, raising the conversion of pyruvate  to oxaloacetate that entries into the Krebs cycle being then oxidized   [57].	transcription
52238	5	334940	5	NULL	NULL	0	NULL	acetyl-CoA	NULL		enhances	NULL				pyruvate carboxylase	NULL	activity of			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1757_1_57_s_240	16375848	Thus, an increase in acetyl-CoA content from palmitate oxidation leads up to inhibition  of pyruvate dehydrogenase activity, decreasing the conversion of pyruvate to acetyl-CoA,  but also enhances pyruvate carboxylase activity, raising the conversion of pyruvate  to oxaloacetate that entries into the Krebs cycle being then oxidized   [57].	transcription
52239	6	334940	5	NULL	NULL	0	NULL	pyruvate	NULL		is converted to	NULL				oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1757_1_57_s_240	16375848	Thus, an increase in acetyl-CoA content from palmitate oxidation leads up to inhibition  of pyruvate dehydrogenase activity, decreasing the conversion of pyruvate to acetyl-CoA,  but also enhances pyruvate carboxylase activity, raising the conversion of pyruvate  to oxaloacetate that entries into the Krebs cycle being then oxidized   [57].	transcription
52240	7	334940	5	NULL	NULL	0	NULL	statement 5	NULL		increases	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1757_1_57_s_240	16375848	Thus, an increase in acetyl-CoA content from palmitate oxidation leads up to inhibition  of pyruvate dehydrogenase activity, decreasing the conversion of pyruvate to acetyl-CoA,  but also enhances pyruvate carboxylase activity, raising the conversion of pyruvate  to oxaloacetate that entries into the Krebs cycle being then oxidized   [57].	transcription
52241	8	334940	5	NULL	NULL	0	NULL	oxaloacetate	NULL		enters into	NULL				Krebs cycle	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1757_1_57_s_240	16375848	Thus, an increase in acetyl-CoA content from palmitate oxidation leads up to inhibition  of pyruvate dehydrogenase activity, decreasing the conversion of pyruvate to acetyl-CoA,  but also enhances pyruvate carboxylase activity, raising the conversion of pyruvate  to oxaloacetate that entries into the Krebs cycle being then oxidized   [57].	transcription
52242	9	334940	5	NULL	NULL	0	NULL	statement 6	NULL		leads to	NULL				statement 8	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1757_1_57_s_240	16375848	Thus, an increase in acetyl-CoA content from palmitate oxidation leads up to inhibition  of pyruvate dehydrogenase activity, decreasing the conversion of pyruvate to acetyl-CoA,  but also enhances pyruvate carboxylase activity, raising the conversion of pyruvate  to oxaloacetate that entries into the Krebs cycle being then oxidized   [57].	transcription
52243	10	334940	5	NULL	NULL	0	NULL	oxaloacetate 	NULL		undergoes	NULL				oxidation	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1757_1_57_s_240	16375848	Thus, an increase in acetyl-CoA content from palmitate oxidation leads up to inhibition  of pyruvate dehydrogenase activity, decreasing the conversion of pyruvate to acetyl-CoA,  but also enhances pyruvate carboxylase activity, raising the conversion of pyruvate  to oxaloacetate that entries into the Krebs cycle being then oxidized   [57].	transcription
52244	11	334940	5	NULL	NULL	0	NULL	statement 8	NULL		leads to	NULL				statement 10	NULL				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1757_1_57_s_240	16375848	Thus, an increase in acetyl-CoA content from palmitate oxidation leads up to inhibition  of pyruvate dehydrogenase activity, decreasing the conversion of pyruvate to acetyl-CoA,  but also enhances pyruvate carboxylase activity, raising the conversion of pyruvate  to oxaloacetate that entries into the Krebs cycle being then oxidized   [57].	transcription
54373	1	334940	6	NULL	NULL	0	NULL	palmitate		oxidation of	increases					acetyl-CoA 		content of 			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1757_1_57_s_240	16375848	Thus, an increase in acetyl-CoA content from palmitate oxidation leads up to inhibition  of pyruvate dehydrogenase activity, decreasing the conversion of pyruvate to acetyl-CoA,  but also enhances pyruvate carboxylase activity, raising the conversion of pyruvate  to oxaloacetate that entries into the Krebs cycle being then oxidized   [57].	transcription
54374	2	334940	6	NULL	NULL	0	NULL	statement 1			leads to					pyruvate dehydrogenase		inhibition of;; activity of			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1757_1_57_s_240	16375848	Thus, an increase in acetyl-CoA content from palmitate oxidation leads up to inhibition  of pyruvate dehydrogenase activity, decreasing the conversion of pyruvate to acetyl-CoA,  but also enhances pyruvate carboxylase activity, raising the conversion of pyruvate  to oxaloacetate that entries into the Krebs cycle being then oxidized   [57].	transcription
54375	3	334940	6	NULL	NULL	0	NULL	pyruvate			is converted to					acetyl-CoA					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1757_1_57_s_240	16375848	Thus, an increase in acetyl-CoA content from palmitate oxidation leads up to inhibition  of pyruvate dehydrogenase activity, decreasing the conversion of pyruvate to acetyl-CoA,  but also enhances pyruvate carboxylase activity, raising the conversion of pyruvate  to oxaloacetate that entries into the Krebs cycle being then oxidized   [57].	transcription
54376	4	334940	6	NULL	NULL	0	NULL	statement 1			decreases					statement 3					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1757_1_57_s_240	16375848	Thus, an increase in acetyl-CoA content from palmitate oxidation leads up to inhibition  of pyruvate dehydrogenase activity, decreasing the conversion of pyruvate to acetyl-CoA,  but also enhances pyruvate carboxylase activity, raising the conversion of pyruvate  to oxaloacetate that entries into the Krebs cycle being then oxidized   [57].	transcription
54377	5	334940	6	NULL	NULL	0	NULL	statement 1			enhances					pyruvate carboxylase		activity of 			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1757_1_57_s_240	16375848	Thus, an increase in acetyl-CoA content from palmitate oxidation leads up to inhibition  of pyruvate dehydrogenase activity, decreasing the conversion of pyruvate to acetyl-CoA,  but also enhances pyruvate carboxylase activity, raising the conversion of pyruvate  to oxaloacetate that entries into the Krebs cycle being then oxidized   [57].	transcription
54378	6	334940	6	NULL	NULL	0	NULL	pyruvate			is converted to					oxaloacetate					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1757_1_57_s_240	16375848	Thus, an increase in acetyl-CoA content from palmitate oxidation leads up to inhibition  of pyruvate dehydrogenase activity, decreasing the conversion of pyruvate to acetyl-CoA,  but also enhances pyruvate carboxylase activity, raising the conversion of pyruvate  to oxaloacetate that entries into the Krebs cycle being then oxidized   [57].	transcription
54379	7	334940	6	NULL	NULL	0	NULL	statement 1			increases					statement 6					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1757_1_57_s_240	16375848	Thus, an increase in acetyl-CoA content from palmitate oxidation leads up to inhibition  of pyruvate dehydrogenase activity, decreasing the conversion of pyruvate to acetyl-CoA,  but also enhances pyruvate carboxylase activity, raising the conversion of pyruvate  to oxaloacetate that entries into the Krebs cycle being then oxidized   [57].	transcription
52245	1	334942	5	NULL	NULL	0	NULL	pyruvate	NULL		enters	NULL				tricarboxylic acid cycle	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_8_2296_s_10	11914362	Pyruvate enters the tricarboxylic acid cycle via the reactions catalyzed by PDH and pyruvate carboxylase (PYC), which are regulated to coordinate the utilization of pyruvate for anabolism (via the anaplerotic production of oxaloacetate by PYC) and catabolism (via acetyl coenzyme A [acetyl-CoA] production by PDH) ( 26).	transcription
52246	2	334942	5	NULL	NULL	0	NULL	statement 1	NULL		via	NULL				PDH	NULL	reactions catalyzed by			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_8_2296_s_10	11914362	Pyruvate enters the tricarboxylic acid cycle via the reactions catalyzed by PDH and pyruvate carboxylase (PYC), which are regulated to coordinate the utilization of pyruvate for anabolism (via the anaplerotic production of oxaloacetate by PYC) and catabolism (via acetyl coenzyme A [acetyl-CoA] production by PDH) ( 26).	transcription
52247	3	334942	5	NULL	NULL	0	NULL	statement 1	NULL		via	NULL				PYC	NULL	reactions catalyzed by			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_8_2296_s_10	11914362	Pyruvate enters the tricarboxylic acid cycle via the reactions catalyzed by PDH and pyruvate carboxylase (PYC), which are regulated to coordinate the utilization of pyruvate for anabolism (via the anaplerotic production of oxaloacetate by PYC) and catabolism (via acetyl coenzyme A [acetyl-CoA] production by PDH) ( 26).	transcription
52248	4	334942	5	NULL	NULL	0	NULL	PYC	NULL		is	NULL				pyruvate carboxylase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_8_2296_s_10	11914362	Pyruvate enters the tricarboxylic acid cycle via the reactions catalyzed by PDH and pyruvate carboxylase (PYC), which are regulated to coordinate the utilization of pyruvate for anabolism (via the anaplerotic production of oxaloacetate by PYC) and catabolism (via acetyl coenzyme A [acetyl-CoA] production by PDH) ( 26).	transcription
52249	5	334942	5	NULL	NULL	0	NULL	pyruvate	NULL		is utilized for	NULL				anabolism	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_8_2296_s_10	11914362	Pyruvate enters the tricarboxylic acid cycle via the reactions catalyzed by PDH and pyruvate carboxylase (PYC), which are regulated to coordinate the utilization of pyruvate for anabolism (via the anaplerotic production of oxaloacetate by PYC) and catabolism (via acetyl coenzyme A [acetyl-CoA] production by PDH) ( 26).	transcription
52250	6	334942	5	NULL	NULL	0	NULL	PYC	NULL		produce	NULL	anaplerotic			oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_8_2296_s_10	11914362	Pyruvate enters the tricarboxylic acid cycle via the reactions catalyzed by PDH and pyruvate carboxylase (PYC), which are regulated to coordinate the utilization of pyruvate for anabolism (via the anaplerotic production of oxaloacetate by PYC) and catabolism (via acetyl coenzyme A [acetyl-CoA] production by PDH) ( 26).	transcription
52251	7	334942	5	NULL	NULL	0	NULL	statement 5	NULL		via	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_8_2296_s_10	11914362	Pyruvate enters the tricarboxylic acid cycle via the reactions catalyzed by PDH and pyruvate carboxylase (PYC), which are regulated to coordinate the utilization of pyruvate for anabolism (via the anaplerotic production of oxaloacetate by PYC) and catabolism (via acetyl coenzyme A [acetyl-CoA] production by PDH) ( 26).	transcription
52252	8	334942	5	NULL	NULL	0	NULL	pyruvate	NULL		is utilized for	NULL				catabolism	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_8_2296_s_10	11914362	Pyruvate enters the tricarboxylic acid cycle via the reactions catalyzed by PDH and pyruvate carboxylase (PYC), which are regulated to coordinate the utilization of pyruvate for anabolism (via the anaplerotic production of oxaloacetate by PYC) and catabolism (via acetyl coenzyme A [acetyl-CoA] production by PDH) ( 26).	transcription
52253	9	334942	5	NULL	NULL	0	NULL	PDH	NULL		produce	NULL				acetyl-CoA	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_8_2296_s_10	11914362	Pyruvate enters the tricarboxylic acid cycle via the reactions catalyzed by PDH and pyruvate carboxylase (PYC), which are regulated to coordinate the utilization of pyruvate for anabolism (via the anaplerotic production of oxaloacetate by PYC) and catabolism (via acetyl coenzyme A [acetyl-CoA] production by PDH) ( 26).	transcription
52254	10	334942	5	NULL	NULL	0	NULL	statement 8	NULL		via	NULL				statement 9	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_8_2296_s_10	11914362	Pyruvate enters the tricarboxylic acid cycle via the reactions catalyzed by PDH and pyruvate carboxylase (PYC), which are regulated to coordinate the utilization of pyruvate for anabolism (via the anaplerotic production of oxaloacetate by PYC) and catabolism (via acetyl coenzyme A [acetyl-CoA] production by PDH) ( 26).	transcription
52255	11	334942	5	NULL	NULL	0	NULL	acetyl-CoA	NULL		is	NULL				acetyl coenzyme A	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_8_2296_s_10	11914362	Pyruvate enters the tricarboxylic acid cycle via the reactions catalyzed by PDH and pyruvate carboxylase (PYC), which are regulated to coordinate the utilization of pyruvate for anabolism (via the anaplerotic production of oxaloacetate by PYC) and catabolism (via acetyl coenzyme A [acetyl-CoA] production by PDH) ( 26).	transcription
52256	12	334942	5	NULL	NULL	0	NULL	PDH	NULL	regulation of	coordinates	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_8_2296_s_10	11914362	Pyruvate enters the tricarboxylic acid cycle via the reactions catalyzed by PDH and pyruvate carboxylase (PYC), which are regulated to coordinate the utilization of pyruvate for anabolism (via the anaplerotic production of oxaloacetate by PYC) and catabolism (via acetyl coenzyme A [acetyl-CoA] production by PDH) ( 26).	transcription
52257	13	334942	5	NULL	NULL	0	NULL	PDH	NULL	regulation of	coordinates	NULL				statement 8	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_8_2296_s_10	11914362	Pyruvate enters the tricarboxylic acid cycle via the reactions catalyzed by PDH and pyruvate carboxylase (PYC), which are regulated to coordinate the utilization of pyruvate for anabolism (via the anaplerotic production of oxaloacetate by PYC) and catabolism (via acetyl coenzyme A [acetyl-CoA] production by PDH) ( 26).	transcription
52258	14	334942	5	NULL	NULL	0	NULL	PYC	NULL	regulation of	coordinates	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_8_2296_s_10	11914362	Pyruvate enters the tricarboxylic acid cycle via the reactions catalyzed by PDH and pyruvate carboxylase (PYC), which are regulated to coordinate the utilization of pyruvate for anabolism (via the anaplerotic production of oxaloacetate by PYC) and catabolism (via acetyl coenzyme A [acetyl-CoA] production by PDH) ( 26).	transcription
52259	15	334942	5	NULL	NULL	0	NULL	PYC	NULL	regulation of	coordinates	NULL				statement 8	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_8_2296_s_10	11914362	Pyruvate enters the tricarboxylic acid cycle via the reactions catalyzed by PDH and pyruvate carboxylase (PYC), which are regulated to coordinate the utilization of pyruvate for anabolism (via the anaplerotic production of oxaloacetate by PYC) and catabolism (via acetyl coenzyme A [acetyl-CoA] production by PDH) ( 26).	transcription
54381	1	334942	6	NULL	NULL	0	NULL	pyruvate			enters 					tricarboxylic acid cycle					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_8_2296_s_10	11914362	Pyruvate enters the tricarboxylic acid cycle via the reactions catalyzed by PDH and pyruvate carboxylase (PYC), which are regulated to coordinate the utilization of pyruvate for anabolism (via the anaplerotic production of oxaloacetate by PYC) and catabolism (via acetyl coenzyme A [acetyl-CoA] production by PDH) ( 26).	transcription
54382	2	334942	6	NULL	NULL	0	NULL	PDH			catalyzes					reactions					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_8_2296_s_10	11914362	Pyruvate enters the tricarboxylic acid cycle via the reactions catalyzed by PDH and pyruvate carboxylase (PYC), which are regulated to coordinate the utilization of pyruvate for anabolism (via the anaplerotic production of oxaloacetate by PYC) and catabolism (via acetyl coenzyme A [acetyl-CoA] production by PDH) ( 26).	transcription
54383	3	334942	6	NULL	NULL	0	NULL	statement 1			occurs via					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_8_2296_s_10	11914362	Pyruvate enters the tricarboxylic acid cycle via the reactions catalyzed by PDH and pyruvate carboxylase (PYC), which are regulated to coordinate the utilization of pyruvate for anabolism (via the anaplerotic production of oxaloacetate by PYC) and catabolism (via acetyl coenzyme A [acetyl-CoA] production by PDH) ( 26).	transcription
54384	4	334942	6	NULL	NULL	0	NULL	PYC			catalyzes					reactions					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_8_2296_s_10	11914362	Pyruvate enters the tricarboxylic acid cycle via the reactions catalyzed by PDH and pyruvate carboxylase (PYC), which are regulated to coordinate the utilization of pyruvate for anabolism (via the anaplerotic production of oxaloacetate by PYC) and catabolism (via acetyl coenzyme A [acetyl-CoA] production by PDH) ( 26).	transcription
54385	5	334942	6	NULL	NULL	0	NULL	statement 4			occurs via					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_8_2296_s_10	11914362	Pyruvate enters the tricarboxylic acid cycle via the reactions catalyzed by PDH and pyruvate carboxylase (PYC), which are regulated to coordinate the utilization of pyruvate for anabolism (via the anaplerotic production of oxaloacetate by PYC) and catabolism (via acetyl coenzyme A [acetyl-CoA] production by PDH) ( 26).	transcription
54386	6	334942	6	NULL	NULL	0	NULL	PYC			produces					oxaloacetate					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_8_2296_s_10	11914362	Pyruvate enters the tricarboxylic acid cycle via the reactions catalyzed by PDH and pyruvate carboxylase (PYC), which are regulated to coordinate the utilization of pyruvate for anabolism (via the anaplerotic production of oxaloacetate by PYC) and catabolism (via acetyl coenzyme A [acetyl-CoA] production by PDH) ( 26).	transcription
54387	7	334942	6	NULL	NULL	0	NULL	statement 6			is					anaplerotic					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_8_2296_s_10	11914362	Pyruvate enters the tricarboxylic acid cycle via the reactions catalyzed by PDH and pyruvate carboxylase (PYC), which are regulated to coordinate the utilization of pyruvate for anabolism (via the anaplerotic production of oxaloacetate by PYC) and catabolism (via acetyl coenzyme A [acetyl-CoA] production by PDH) ( 26).	transcription
54388	8	334942	6	NULL	NULL	0	NULL	PDH			produces					acetyl-CoA					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_8_2296_s_10	11914362	Pyruvate enters the tricarboxylic acid cycle via the reactions catalyzed by PDH and pyruvate carboxylase (PYC), which are regulated to coordinate the utilization of pyruvate for anabolism (via the anaplerotic production of oxaloacetate by PYC) and catabolism (via acetyl coenzyme A [acetyl-CoA] production by PDH) ( 26).	transcription
54389	9	334942	6	NULL	NULL	0	NULL	acetyl-CoA			is					acetyl coenzyme A					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_8_2296_s_10	11914362	Pyruvate enters the tricarboxylic acid cycle via the reactions catalyzed by PDH and pyruvate carboxylase (PYC), which are regulated to coordinate the utilization of pyruvate for anabolism (via the anaplerotic production of oxaloacetate by PYC) and catabolism (via acetyl coenzyme A [acetyl-CoA] production by PDH) ( 26).	transcription
52260	1	334943	5	NULL	NULL	0	NULL	oxaloacetate	NULL		is diverted from	NULL				phosphoenolpyruvate	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_8_4705_s_229	9030522	Table  VIII also shows that the acetate-induced diversion of oxaloacetate from phosphoenolpyruvate formation to citrate synthesis was logically accompanied by a large decrease in flux through pyruvate kinase and therefore in a decreased availability of pyruvate leading to a diminution of fluxes through alanine aminotransferase and pyruvate dehydrogenase.	transcription
52261	2	334943	5	NULL	NULL	0	NULL	oxaloacetate	NULL		is diverted to	NULL				citrate	NULL	synthesis of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_8_4705_s_229	9030522	Table  VIII also shows that the acetate-induced diversion of oxaloacetate from phosphoenolpyruvate formation to citrate synthesis was logically accompanied by a large decrease in flux through pyruvate kinase and therefore in a decreased availability of pyruvate leading to a diminution of fluxes through alanine aminotransferase and pyruvate dehydrogenase.	transcription
52262	3	334943	5	NULL	NULL	0	NULL	acetate	NULL		induce	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_8_4705_s_229	9030522	Table  VIII also shows that the acetate-induced diversion of oxaloacetate from phosphoenolpyruvate formation to citrate synthesis was logically accompanied by a large decrease in flux through pyruvate kinase and therefore in a decreased availability of pyruvate leading to a diminution of fluxes through alanine aminotransferase and pyruvate dehydrogenase.	transcription
52263	4	334943	5	NULL	NULL	0	NULL	acetate	NULL		induce	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_8_4705_s_229	9030522	Table  VIII also shows that the acetate-induced diversion of oxaloacetate from phosphoenolpyruvate formation to citrate synthesis was logically accompanied by a large decrease in flux through pyruvate kinase and therefore in a decreased availability of pyruvate leading to a diminution of fluxes through alanine aminotransferase and pyruvate dehydrogenase.	transcription
52264	5	334943	5	NULL	NULL	0	NULL	flux	NULL	decrease in	occurs through	NULL				pyruvate kinase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_8_4705_s_229	9030522	Table  VIII also shows that the acetate-induced diversion of oxaloacetate from phosphoenolpyruvate formation to citrate synthesis was logically accompanied by a large decrease in flux through pyruvate kinase and therefore in a decreased availability of pyruvate leading to a diminution of fluxes through alanine aminotransferase and pyruvate dehydrogenase.	transcription
52265	6	334943	5	NULL	NULL	0	NULL	statement 4	NULL		is accompanied by	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_8_4705_s_229	9030522	Table  VIII also shows that the acetate-induced diversion of oxaloacetate from phosphoenolpyruvate formation to citrate synthesis was logically accompanied by a large decrease in flux through pyruvate kinase and therefore in a decreased availability of pyruvate leading to a diminution of fluxes through alanine aminotransferase and pyruvate dehydrogenase.	transcription
52266	7	334943	5	NULL	NULL	0	NULL	statement 6	NULL		leads to	NULL				pyruvate	NULL	decreased availability of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_8_4705_s_229	9030522	Table  VIII also shows that the acetate-induced diversion of oxaloacetate from phosphoenolpyruvate formation to citrate synthesis was logically accompanied by a large decrease in flux through pyruvate kinase and therefore in a decreased availability of pyruvate leading to a diminution of fluxes through alanine aminotransferase and pyruvate dehydrogenase.	transcription
52267	8	334943	5	NULL	NULL	0	NULL	statement 7	NULL		leads to	NULL				fluxes	NULL	diminution of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_8_4705_s_229	9030522	Table  VIII also shows that the acetate-induced diversion of oxaloacetate from phosphoenolpyruvate formation to citrate synthesis was logically accompanied by a large decrease in flux through pyruvate kinase and therefore in a decreased availability of pyruvate leading to a diminution of fluxes through alanine aminotransferase and pyruvate dehydrogenase.	transcription
52268	9	334943	5	NULL	NULL	0	NULL	statement 8	NULL		occurs through	NULL				alanine aminotransferase 	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_8_4705_s_229	9030522	Table  VIII also shows that the acetate-induced diversion of oxaloacetate from phosphoenolpyruvate formation to citrate synthesis was logically accompanied by a large decrease in flux through pyruvate kinase and therefore in a decreased availability of pyruvate leading to a diminution of fluxes through alanine aminotransferase and pyruvate dehydrogenase.	transcription
52269	10	334943	5	NULL	NULL	0	NULL	statement 8	NULL		occurs through	NULL				pyruvate dehydrogenase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_8_4705_s_229	9030522	Table  VIII also shows that the acetate-induced diversion of oxaloacetate from phosphoenolpyruvate formation to citrate synthesis was logically accompanied by a large decrease in flux through pyruvate kinase and therefore in a decreased availability of pyruvate leading to a diminution of fluxes through alanine aminotransferase and pyruvate dehydrogenase.	transcription
55616	1	334943	6	NULL	NULL	0	NULL	oxaloacetate			forms					phosphoenolpyruvate					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_8_4705_s_229	9030522	Table  VIII also shows that the acetate-induced diversion of oxaloacetate from phosphoenolpyruvate formation to citrate synthesis was logically accompanied by a large decrease in flux through pyruvate kinase and therefore in a decreased availability of pyruvate leading to a diminution of fluxes through alanine aminotransferase and pyruvate dehydrogenase.	transcription
55617	2	334943	6	NULL	NULL	0	NULL	oxaloacetate			forms					citrate					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_8_4705_s_229	9030522	Table  VIII also shows that the acetate-induced diversion of oxaloacetate from phosphoenolpyruvate formation to citrate synthesis was logically accompanied by a large decrease in flux through pyruvate kinase and therefore in a decreased availability of pyruvate leading to a diminution of fluxes through alanine aminotransferase and pyruvate dehydrogenase.	transcription
55618	3	334943	6	NULL	NULL	0	NULL	acetate			induces					oxaloacetate		diversion of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_8_4705_s_229	9030522	Table  VIII also shows that the acetate-induced diversion of oxaloacetate from phosphoenolpyruvate formation to citrate synthesis was logically accompanied by a large decrease in flux through pyruvate kinase and therefore in a decreased availability of pyruvate leading to a diminution of fluxes through alanine aminotransferase and pyruvate dehydrogenase.	transcription
55619	4	334943	6	NULL	NULL	0	NULL	statement 3			allows					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_8_4705_s_229	9030522	Table  VIII also shows that the acetate-induced diversion of oxaloacetate from phosphoenolpyruvate formation to citrate synthesis was logically accompanied by a large decrease in flux through pyruvate kinase and therefore in a decreased availability of pyruvate leading to a diminution of fluxes through alanine aminotransferase and pyruvate dehydrogenase.	transcription
52270	1	334944	5	NULL	NULL	0	NULL	5S	NULL		is a type of	NULL				120 kDa dimer	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevphyschem_57_0_527_s_306	16599820	In  2000 our laboratory began Raman crystallographic studies on transcarboxylase's  second major subunit, the so-called 5S, a 120 kDa dimer that converts bound pyruvate  to oxaloacetate using -CO2  from carboxybiotin ( 21).	transcription
52271	2	334944	5	NULL	NULL	0	NULL	5S	NULL		is a subunit of	NULL	major			transcarboxylase	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevphyschem_57_0_527_s_306	16599820	In  2000 our laboratory began Raman crystallographic studies on transcarboxylase's  second major subunit, the so-called 5S, a 120 kDa dimer that converts bound pyruvate  to oxaloacetate using -CO2  from carboxybiotin ( 21).	transcription
52272	3	334944	5	NULL	NULL	0	NULL	pyruvate	NULL	bound	is converted to	NULL				oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevphyschem_57_0_527_s_306	16599820	In  2000 our laboratory began Raman crystallographic studies on transcarboxylase's  second major subunit, the so-called 5S, a 120 kDa dimer that converts bound pyruvate  to oxaloacetate using -CO2  from carboxybiotin ( 21).	transcription
52273	4	334944	5	NULL	NULL	0	NULL	transcarboxylase	NULL		catalyzes	NULL		5S		statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_annurevphyschem_57_0_527_s_306	16599820	In  2000 our laboratory began Raman crystallographic studies on transcarboxylase's  second major subunit, the so-called 5S, a 120 kDa dimer that converts bound pyruvate  to oxaloacetate using -CO2  from carboxybiotin ( 21).	transcription
52274	5	334944	5	NULL	NULL	0	NULL	statement 4	NULL		uses	NULL				carboxybiotin	NULL		-CO2		NULL		0	NULL	NULL	NULL	gw70_annurevphyschem_57_0_527_s_306	16599820	In  2000 our laboratory began Raman crystallographic studies on transcarboxylase's  second major subunit, the so-called 5S, a 120 kDa dimer that converts bound pyruvate  to oxaloacetate using -CO2  from carboxybiotin ( 21).	transcription
54390	1	334944	6	NULL	NULL	0	NULL	pyruvate			is converted to					oxaloacetate					NULL		0	NULL	NULL	NULL	gw70_annurevphyschem_57_0_527_s_306	16599820	In  2000 our laboratory began Raman crystallographic studies on transcarboxylase's  second major subunit, the so-called 5S, a 120 kDa dimer that converts bound pyruvate  to oxaloacetate using -CO2  from carboxybiotin ( 21).	transcription
54391	2	334944	6	NULL	NULL	0	NULL	5S subunit			converts					statement 1					NULL		0	NULL	NULL	NULL	gw70_annurevphyschem_57_0_527_s_306	16599820	In  2000 our laboratory began Raman crystallographic studies on transcarboxylase's  second major subunit, the so-called 5S, a 120 kDa dimer that converts bound pyruvate  to oxaloacetate using -CO2  from carboxybiotin ( 21).	transcription
54392	3	334944	6	NULL	NULL	0	NULL	5S subunit			is					transcarboxylase second major subunit					NULL		0	NULL	NULL	NULL	gw70_annurevphyschem_57_0_527_s_306	16599820	In  2000 our laboratory began Raman crystallographic studies on transcarboxylase's  second major subunit, the so-called 5S, a 120 kDa dimer that converts bound pyruvate  to oxaloacetate using -CO2  from carboxybiotin ( 21).	transcription
54393	4	334944	6	NULL	NULL	0	NULL	CO2			is used from					carboxybiotin					NULL		0	NULL	NULL	NULL	gw70_annurevphyschem_57_0_527_s_306	16599820	In  2000 our laboratory began Raman crystallographic studies on transcarboxylase's  second major subunit, the so-called 5S, a 120 kDa dimer that converts bound pyruvate  to oxaloacetate using -CO2  from carboxybiotin ( 21).	transcription
54394	5	334944	6	NULL	NULL	0	NULL	statement 1			occurs via					statement 4					NULL		0	NULL	NULL	NULL	gw70_annurevphyschem_57_0_527_s_306	16599820	In  2000 our laboratory began Raman crystallographic studies on transcarboxylase's  second major subunit, the so-called 5S, a 120 kDa dimer that converts bound pyruvate  to oxaloacetate using -CO2  from carboxybiotin ( 21).	transcription
52275	1	334945	5	NULL	NULL	0	NULL	U251-HRE cells	NULL		is	NULL				U251 cells stably expressing (HRE)-luciferase construct	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_126	16223732	Using U251 cells stably expressing a hypoxia regulatory element (HRE)-luciferase construct (U251-HRE cells;  Fig. 1 E), we found that pyruvate and oxaloacetate induced the HIF-1-regulated reporter gene as effectively as hypoxia or DMOG.	transcription
52276	2	334945	5	NULL	NULL	0	NULL	HRE	NULL		is	NULL				hypoxia regulatory element	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_126	16223732	Using U251 cells stably expressing a hypoxia regulatory element (HRE)-luciferase construct (U251-HRE cells;  Fig. 1 E), we found that pyruvate and oxaloacetate induced the HIF-1-regulated reporter gene as effectively as hypoxia or DMOG.	transcription
52277	3	334945	5	NULL	NULL	0	NULL	reporter gene	NULL		is regulated by	NULL				HIF-1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_126	16223732	Using U251 cells stably expressing a hypoxia regulatory element (HRE)-luciferase construct (U251-HRE cells;  Fig. 1 E), we found that pyruvate and oxaloacetate induced the HIF-1-regulated reporter gene as effectively as hypoxia or DMOG.	transcription
52278	4	334945	5	NULL	NULL	0	NULL	pyruvate	NULL		induce	NULL				statement 3	NULL				NULL	U251-HRE cells	0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_126	16223732	Using U251 cells stably expressing a hypoxia regulatory element (HRE)-luciferase construct (U251-HRE cells;  Fig. 1 E), we found that pyruvate and oxaloacetate induced the HIF-1-regulated reporter gene as effectively as hypoxia or DMOG.	transcription
52279	5	334945	5	NULL	NULL	0	NULL	oxaloacetate	NULL		induce	NULL				statement 3	NULL				NULL	U251-HRE cells	0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_126	16223732	Using U251 cells stably expressing a hypoxia regulatory element (HRE)-luciferase construct (U251-HRE cells;  Fig. 1 E), we found that pyruvate and oxaloacetate induced the HIF-1-regulated reporter gene as effectively as hypoxia or DMOG.	transcription
52280	6	334945	5	NULL	NULL	0	NULL	hypoxia	NULL		induce	NULL				statement 3	NULL				NULL	U251-HRE cells	0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_126	16223732	Using U251 cells stably expressing a hypoxia regulatory element (HRE)-luciferase construct (U251-HRE cells;  Fig. 1 E), we found that pyruvate and oxaloacetate induced the HIF-1-regulated reporter gene as effectively as hypoxia or DMOG.	transcription
52281	7	334945	5	NULL	NULL	0	NULL	DMOG	NULL		induce	NULL				statement 3	NULL				NULL	U251-HRE cells	0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_126	16223732	Using U251 cells stably expressing a hypoxia regulatory element (HRE)-luciferase construct (U251-HRE cells;  Fig. 1 E), we found that pyruvate and oxaloacetate induced the HIF-1-regulated reporter gene as effectively as hypoxia or DMOG.	transcription
52282	8	334945	5	NULL	NULL	0	NULL	statement 4	NULL		as effecective as	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_126	16223732	Using U251 cells stably expressing a hypoxia regulatory element (HRE)-luciferase construct (U251-HRE cells;  Fig. 1 E), we found that pyruvate and oxaloacetate induced the HIF-1-regulated reporter gene as effectively as hypoxia or DMOG.	transcription
52283	9	334945	5	NULL	NULL	0	NULL	statement 5	NULL		as effecective as	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_126	16223732	Using U251 cells stably expressing a hypoxia regulatory element (HRE)-luciferase construct (U251-HRE cells;  Fig. 1 E), we found that pyruvate and oxaloacetate induced the HIF-1-regulated reporter gene as effectively as hypoxia or DMOG.	transcription
52284	10	334945	5	NULL	NULL	0	NULL	statement 4	NULL		as effecective as	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_126	16223732	Using U251 cells stably expressing a hypoxia regulatory element (HRE)-luciferase construct (U251-HRE cells;  Fig. 1 E), we found that pyruvate and oxaloacetate induced the HIF-1-regulated reporter gene as effectively as hypoxia or DMOG.	transcription
52285	11	334945	5	NULL	NULL	0	NULL	statement 5	NULL		as effecective as	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_126	16223732	Using U251 cells stably expressing a hypoxia regulatory element (HRE)-luciferase construct (U251-HRE cells;  Fig. 1 E), we found that pyruvate and oxaloacetate induced the HIF-1-regulated reporter gene as effectively as hypoxia or DMOG.	transcription
54395	1	334945	6	NULL	NULL	0	NULL	HIF			regulates					reporter gene					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_126	16223732	Using U251 cells stably expressing a hypoxia regulatory element (HRE)-luciferase construct (U251-HRE cells;  Fig. 1 E), we found that pyruvate and oxaloacetate induced the HIF-1-regulated reporter gene as effectively as hypoxia or DMOG.	transcription
54396	2	334945	6	NULL	NULL	0	NULL	pyruvate			induces					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_126	16223732	Using U251 cells stably expressing a hypoxia regulatory element (HRE)-luciferase construct (U251-HRE cells;  Fig. 1 E), we found that pyruvate and oxaloacetate induced the HIF-1-regulated reporter gene as effectively as hypoxia or DMOG.	transcription
54397	3	334945	6	NULL	NULL	0	NULL	oxaloacetate			induces					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_126	16223732	Using U251 cells stably expressing a hypoxia regulatory element (HRE)-luciferase construct (U251-HRE cells;  Fig. 1 E), we found that pyruvate and oxaloacetate induced the HIF-1-regulated reporter gene as effectively as hypoxia or DMOG.	transcription
54398	4	334945	6	NULL	NULL	0	NULL	hypoxia			induces					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_126	16223732	Using U251 cells stably expressing a hypoxia regulatory element (HRE)-luciferase construct (U251-HRE cells;  Fig. 1 E), we found that pyruvate and oxaloacetate induced the HIF-1-regulated reporter gene as effectively as hypoxia or DMOG.	transcription
54399	5	334945	6	NULL	NULL	0	NULL	DMOG			induces					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_126	16223732	Using U251 cells stably expressing a hypoxia regulatory element (HRE)-luciferase construct (U251-HRE cells;  Fig. 1 E), we found that pyruvate and oxaloacetate induced the HIF-1-regulated reporter gene as effectively as hypoxia or DMOG.	transcription
54400	6	334945	6	NULL	NULL	0	NULL	statement 4			is an alternative to					statement 5					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_126	16223732	Using U251 cells stably expressing a hypoxia regulatory element (HRE)-luciferase construct (U251-HRE cells;  Fig. 1 E), we found that pyruvate and oxaloacetate induced the HIF-1-regulated reporter gene as effectively as hypoxia or DMOG.	transcription
52286	1	334946	5	NULL	NULL	0	NULL	2-oxoacids	NULL		induce	NULL				HIF-1 gene	NULL			reporter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_128	16223732	Induction of the HIF-1 reporter gene by the 2-oxoacids was also selectively reversed by ascorbate but not by 2-OG. Ascorbate did not reverse HRE-luciferase activation by hypoxia or by DMOG, again suggesting a unique mode of HIF-1alpha regulation by pyruvate and oxaloacetate.	transcription
52287	2	334946	5	NULL	NULL	0	NULL	statement 1	NULL		is reversed by	NULL	selectively			ascorbate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_128	16223732	Induction of the HIF-1 reporter gene by the 2-oxoacids was also selectively reversed by ascorbate but not by 2-OG. Ascorbate did not reverse HRE-luciferase activation by hypoxia or by DMOG, again suggesting a unique mode of HIF-1alpha regulation by pyruvate and oxaloacetate.	transcription
52288	3	334946	5	NULL	NULL	0	NULL	statement 1	NULL		is not reversed by	NULL				2-OG	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_128	16223732	Induction of the HIF-1 reporter gene by the 2-oxoacids was also selectively reversed by ascorbate but not by 2-OG. Ascorbate did not reverse HRE-luciferase activation by hypoxia or by DMOG, again suggesting a unique mode of HIF-1alpha regulation by pyruvate and oxaloacetate.	transcription
52289	4	334946	5	NULL	NULL	0	NULL	HIF-1alpha	NULL		is regulated by	NULL				pyruvate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_128	16223732	Induction of the HIF-1 reporter gene by the 2-oxoacids was also selectively reversed by ascorbate but not by 2-OG. Ascorbate did not reverse HRE-luciferase activation by hypoxia or by DMOG, again suggesting a unique mode of HIF-1alpha regulation by pyruvate and oxaloacetate.	transcription
52290	5	334946	5	NULL	NULL	0	NULL	HIF-1alpha	NULL		is regulated by	NULL				oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_128	16223732	Induction of the HIF-1 reporter gene by the 2-oxoacids was also selectively reversed by ascorbate but not by 2-OG. Ascorbate did not reverse HRE-luciferase activation by hypoxia or by DMOG, again suggesting a unique mode of HIF-1alpha regulation by pyruvate and oxaloacetate.	transcription
52291	6	334946	5	NULL	NULL	0	NULL	hypoxia	NULL		activates	NULL				HRE-luciferase	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_128	16223732	Induction of the HIF-1 reporter gene by the 2-oxoacids was also selectively reversed by ascorbate but not by 2-OG. Ascorbate did not reverse HRE-luciferase activation by hypoxia or by DMOG, again suggesting a unique mode of HIF-1alpha regulation by pyruvate and oxaloacetate.	transcription
52292	7	334946	5	NULL	NULL	0	NULL	DMOG	NULL		activates	NULL				HRE-luciferase	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_128	16223732	Induction of the HIF-1 reporter gene by the 2-oxoacids was also selectively reversed by ascorbate but not by 2-OG. Ascorbate did not reverse HRE-luciferase activation by hypoxia or by DMOG, again suggesting a unique mode of HIF-1alpha regulation by pyruvate and oxaloacetate.	transcription
52293	8	334946	5	NULL	NULL	0	NULL	ascorbate	NULL		does not reverse	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_128	16223732	Induction of the HIF-1 reporter gene by the 2-oxoacids was also selectively reversed by ascorbate but not by 2-OG. Ascorbate did not reverse HRE-luciferase activation by hypoxia or by DMOG, again suggesting a unique mode of HIF-1alpha regulation by pyruvate and oxaloacetate.	transcription
52294	9	334946	5	NULL	NULL	0	NULL	ascorbate	NULL		does not reverse	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_128	16223732	Induction of the HIF-1 reporter gene by the 2-oxoacids was also selectively reversed by ascorbate but not by 2-OG. Ascorbate did not reverse HRE-luciferase activation by hypoxia or by DMOG, again suggesting a unique mode of HIF-1alpha regulation by pyruvate and oxaloacetate.	transcription
79259	1	334946	6	NULL	NULL	0	NULL	2-oxoacids	Chemical		induces					HIF-1 gene					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_128	16223732	Induction of the HIF-1 reporter gene by the 2-oxoacids was also selectively reversed by ascorbate but not by 2-OG. Ascorbate did not reverse HRE-luciferase activation by hypoxia or by DMOG, again suggesting a unique mode of HIF-1alpha regulation by pyruvate and oxaloacetate.	transcription
79260	2	334946	6	NULL	NULL	0	NULL	ascorbate	Chemical		reverses					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_128	16223732	Induction of the HIF-1 reporter gene by the 2-oxoacids was also selectively reversed by ascorbate but not by 2-OG. Ascorbate did not reverse HRE-luciferase activation by hypoxia or by DMOG, again suggesting a unique mode of HIF-1alpha regulation by pyruvate and oxaloacetate.	transcription
52295	1	334947	5	NULL	NULL	0	NULL	HIF-1alpha	NULL		is induced by	NULL				pyruvate	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_154	16223732	Pharmacological inhibition of other signaling pathways implicated in HIF-1alpha stabilization, such as protein acetylation, phosphatidylinositol 3-kinase, mTOR, and hsp70, also failed to alter HIF-1alpha induction by pyruvate and oxaloacetate ( Fig. 3 C).	transcription
52296	2	334947	5	NULL	NULL	0	NULL	HIF-1alpha	NULL		is induced by	NULL				oxaloacetate	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_154	16223732	Pharmacological inhibition of other signaling pathways implicated in HIF-1alpha stabilization, such as protein acetylation, phosphatidylinositol 3-kinase, mTOR, and hsp70, also failed to alter HIF-1alpha induction by pyruvate and oxaloacetate ( Fig. 3 C).	transcription
52297	3	334947	5	NULL	NULL	0	NULL	protein	NULL	acetylation of	is implicated in	NULL				HIF-1alpha	NULL	stabilization of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_154	16223732	Pharmacological inhibition of other signaling pathways implicated in HIF-1alpha stabilization, such as protein acetylation, phosphatidylinositol 3-kinase, mTOR, and hsp70, also failed to alter HIF-1alpha induction by pyruvate and oxaloacetate ( Fig. 3 C).	transcription
52298	4	334947	5	NULL	NULL	0	NULL	protein	NULL	inhibition of;;acetylation of	does not alter	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_154	16223732	Pharmacological inhibition of other signaling pathways implicated in HIF-1alpha stabilization, such as protein acetylation, phosphatidylinositol 3-kinase, mTOR, and hsp70, also failed to alter HIF-1alpha induction by pyruvate and oxaloacetate ( Fig. 3 C).	transcription
52299	5	334947	5	NULL	NULL	0	NULL	protein	NULL	inhibition of;;acetylation of	does not alter	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_154	16223732	Pharmacological inhibition of other signaling pathways implicated in HIF-1alpha stabilization, such as protein acetylation, phosphatidylinositol 3-kinase, mTOR, and hsp70, also failed to alter HIF-1alpha induction by pyruvate and oxaloacetate ( Fig. 3 C).	transcription
52300	6	334947	5	NULL	NULL	0	NULL	phosphatidylinositol 3-kinase	NULL		is implicated in	NULL				HIF-1alpha	NULL	stabilization of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_154	16223732	Pharmacological inhibition of other signaling pathways implicated in HIF-1alpha stabilization, such as protein acetylation, phosphatidylinositol 3-kinase, mTOR, and hsp70, also failed to alter HIF-1alpha induction by pyruvate and oxaloacetate ( Fig. 3 C).	transcription
52301	7	334947	5	NULL	NULL	0	NULL	phosphatidylinositol 3-kinase	NULL	inhibition of	does not alter	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_154	16223732	Pharmacological inhibition of other signaling pathways implicated in HIF-1alpha stabilization, such as protein acetylation, phosphatidylinositol 3-kinase, mTOR, and hsp70, also failed to alter HIF-1alpha induction by pyruvate and oxaloacetate ( Fig. 3 C).	transcription
52302	8	334947	5	NULL	NULL	0	NULL	phosphatidylinositol 3-kinase	NULL	inhibition of	does not alter	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_154	16223732	Pharmacological inhibition of other signaling pathways implicated in HIF-1alpha stabilization, such as protein acetylation, phosphatidylinositol 3-kinase, mTOR, and hsp70, also failed to alter HIF-1alpha induction by pyruvate and oxaloacetate ( Fig. 3 C).	transcription
52303	9	334947	5	NULL	NULL	0	NULL	mTOR	NULL		is implicated in	NULL				HIF-1alpha	NULL	stabilization of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_154	16223732	Pharmacological inhibition of other signaling pathways implicated in HIF-1alpha stabilization, such as protein acetylation, phosphatidylinositol 3-kinase, mTOR, and hsp70, also failed to alter HIF-1alpha induction by pyruvate and oxaloacetate ( Fig. 3 C).	transcription
52304	10	334947	5	NULL	NULL	0	NULL	mTOR	NULL	inhibition of	does not alter	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_154	16223732	Pharmacological inhibition of other signaling pathways implicated in HIF-1alpha stabilization, such as protein acetylation, phosphatidylinositol 3-kinase, mTOR, and hsp70, also failed to alter HIF-1alpha induction by pyruvate and oxaloacetate ( Fig. 3 C).	transcription
52305	11	334947	5	NULL	NULL	0	NULL	mTOR	NULL	inhibition of	does not alter	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_154	16223732	Pharmacological inhibition of other signaling pathways implicated in HIF-1alpha stabilization, such as protein acetylation, phosphatidylinositol 3-kinase, mTOR, and hsp70, also failed to alter HIF-1alpha induction by pyruvate and oxaloacetate ( Fig. 3 C).	transcription
52306	12	334947	5	NULL	NULL	0	NULL	hsp70	NULL		is implicated in	NULL				HIF-1alpha	NULL	stabilization of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_154	16223732	Pharmacological inhibition of other signaling pathways implicated in HIF-1alpha stabilization, such as protein acetylation, phosphatidylinositol 3-kinase, mTOR, and hsp70, also failed to alter HIF-1alpha induction by pyruvate and oxaloacetate ( Fig. 3 C).	transcription
52307	13	334947	5	NULL	NULL	0	NULL	hsp70	NULL	inhibition of	does not alter	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_154	16223732	Pharmacological inhibition of other signaling pathways implicated in HIF-1alpha stabilization, such as protein acetylation, phosphatidylinositol 3-kinase, mTOR, and hsp70, also failed to alter HIF-1alpha induction by pyruvate and oxaloacetate ( Fig. 3 C).	transcription
52308	14	334947	5	NULL	NULL	0	NULL	hsp70	NULL	inhibition of	does not alter	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_154	16223732	Pharmacological inhibition of other signaling pathways implicated in HIF-1alpha stabilization, such as protein acetylation, phosphatidylinositol 3-kinase, mTOR, and hsp70, also failed to alter HIF-1alpha induction by pyruvate and oxaloacetate ( Fig. 3 C).	transcription
54401	1	334947	6	NULL	NULL	0	NULL	pyruvate			induces					HIF-1alpha		induction of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_154	16223732	Pharmacological inhibition of other signaling pathways implicated in HIF-1alpha stabilization, such as protein acetylation, phosphatidylinositol 3-kinase, mTOR, and hsp70, also failed to alter HIF-1alpha induction by pyruvate and oxaloacetate ( Fig. 3 C).	transcription
54402	2	334947	6	NULL	NULL	0	NULL	oxaloacetate			induces					HIF-1alpha		induction of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_154	16223732	Pharmacological inhibition of other signaling pathways implicated in HIF-1alpha stabilization, such as protein acetylation, phosphatidylinositol 3-kinase, mTOR, and hsp70, also failed to alter HIF-1alpha induction by pyruvate and oxaloacetate ( Fig. 3 C).	transcription
54403	3	334947	6	NULL	NULL	0	NULL	phosphatidylinositol 3-kinase		inhibition of 	does not alter					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_154	16223732	Pharmacological inhibition of other signaling pathways implicated in HIF-1alpha stabilization, such as protein acetylation, phosphatidylinositol 3-kinase, mTOR, and hsp70, also failed to alter HIF-1alpha induction by pyruvate and oxaloacetate ( Fig. 3 C).	transcription
54404	4	334947	6	NULL	NULL	0	NULL	phosphatidylinositol 3-kinase		inhibition of 	does not alter					statement 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_154	16223732	Pharmacological inhibition of other signaling pathways implicated in HIF-1alpha stabilization, such as protein acetylation, phosphatidylinositol 3-kinase, mTOR, and hsp70, also failed to alter HIF-1alpha induction by pyruvate and oxaloacetate ( Fig. 3 C).	transcription
54405	5	334947	6	NULL	NULL	0	NULL	mTOR		inhibition of 	does not alter					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_154	16223732	Pharmacological inhibition of other signaling pathways implicated in HIF-1alpha stabilization, such as protein acetylation, phosphatidylinositol 3-kinase, mTOR, and hsp70, also failed to alter HIF-1alpha induction by pyruvate and oxaloacetate ( Fig. 3 C).	transcription
54406	6	334947	6	NULL	NULL	0	NULL	mTOR		inhibition of 	does not alter					statement 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_154	16223732	Pharmacological inhibition of other signaling pathways implicated in HIF-1alpha stabilization, such as protein acetylation, phosphatidylinositol 3-kinase, mTOR, and hsp70, also failed to alter HIF-1alpha induction by pyruvate and oxaloacetate ( Fig. 3 C).	transcription
54407	7	334947	6	NULL	NULL	0	NULL	hsp70		inhibition of 	does not alter					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_154	16223732	Pharmacological inhibition of other signaling pathways implicated in HIF-1alpha stabilization, such as protein acetylation, phosphatidylinositol 3-kinase, mTOR, and hsp70, also failed to alter HIF-1alpha induction by pyruvate and oxaloacetate ( Fig. 3 C).	transcription
54408	8	334947	6	NULL	NULL	0	NULL	hsp70		inhibition of 	does not alter					statement 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_154	16223732	Pharmacological inhibition of other signaling pathways implicated in HIF-1alpha stabilization, such as protein acetylation, phosphatidylinositol 3-kinase, mTOR, and hsp70, also failed to alter HIF-1alpha induction by pyruvate and oxaloacetate ( Fig. 3 C).	transcription
52309	1	334948	5	NULL	NULL	0	NULL	HPH1	NULL	in vitro translated	hydroxylates	NULL				HIF-1alpha peptide	NULL	biotinylated	Pro564		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_201	16223732	To determine whether HPH activity was directly modulated by pyruvate or oxaloacetate, we studied Pro564 hydroxylation in a biotinylated HIF-1alpha ODD peptide by  in vitro translated HPH1, HPH2, and HPH3.	transcription
52310	2	334948	5	NULL	NULL	0	NULL	HPH2	NULL	in vitro translated	hydroxylates	NULL				HIF-1alpha peptide	NULL	biotinylated	Pro564		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_201	16223732	To determine whether HPH activity was directly modulated by pyruvate or oxaloacetate, we studied Pro564 hydroxylation in a biotinylated HIF-1alpha ODD peptide by  in vitro translated HPH1, HPH2, and HPH3.	transcription
52311	3	334948	5	NULL	NULL	0	NULL	HPH3	NULL	in vitro translated	hydroxylates	NULL				HIF-1alpha peptide	NULL	biotinylated	Pro564		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_51_41928_s_201	16223732	To determine whether HPH activity was directly modulated by pyruvate or oxaloacetate, we studied Pro564 hydroxylation in a biotinylated HIF-1alpha ODD peptide by  in vitro translated HPH1, HPH2, and HPH3.	transcription
52312	1	334951	5	NULL	NULL	0	NULL	protocatechuate	NULL		is converted to	NULL				pyruvate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_12_3689_s_308	11371533	It is not required for the conversion of protocatechuate to pyruvate and oxaloacetate (above), and extracts of  E. coli strains carrying the  pcmF gene (on pRE1056, e.g.) did not have activity toward such substrates as 2-hydroxy-4-carboxymuconic semialdehyde and 2-pyrone-4,6-dicarboxylate.	transcription
52313	2	334951	5	NULL	NULL	0	NULL	protocatechuate	NULL		is converted to	NULL				oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_12_3689_s_308	11371533	It is not required for the conversion of protocatechuate to pyruvate and oxaloacetate (above), and extracts of  E. coli strains carrying the  pcmF gene (on pRE1056, e.g.) did not have activity toward such substrates as 2-hydroxy-4-carboxymuconic semialdehyde and 2-pyrone-4,6-dicarboxylate.	transcription
52314	3	334951	5	NULL	NULL	0	NULL	statement 1	NULL		occurs along with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_12_3689_s_308	11371533	It is not required for the conversion of protocatechuate to pyruvate and oxaloacetate (above), and extracts of  E. coli strains carrying the  pcmF gene (on pRE1056, e.g.) did not have activity toward such substrates as 2-hydroxy-4-carboxymuconic semialdehyde and 2-pyrone-4,6-dicarboxylate.	transcription
52315	4	334951	5	NULL	NULL	0	NULL	E. coli strains	NULL	extracts of	carries	NULL				pcmF gene	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_12_3689_s_308	11371533	It is not required for the conversion of protocatechuate to pyruvate and oxaloacetate (above), and extracts of  E. coli strains carrying the  pcmF gene (on pRE1056, e.g.) did not have activity toward such substrates as 2-hydroxy-4-carboxymuconic semialdehyde and 2-pyrone-4,6-dicarboxylate.	transcription
52316	5	334951	5	NULL	NULL	0	NULL	statement 4	NULL		does have activity towards	NULL				2-hydroxy-4-carboxymuconic semialdehyde	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_12_3689_s_308	11371533	It is not required for the conversion of protocatechuate to pyruvate and oxaloacetate (above), and extracts of  E. coli strains carrying the  pcmF gene (on pRE1056, e.g.) did not have activity toward such substrates as 2-hydroxy-4-carboxymuconic semialdehyde and 2-pyrone-4,6-dicarboxylate.	transcription
52317	6	334951	5	NULL	NULL	0	NULL	statement 4	NULL		does have activity towards	NULL				2-pyrone-4,6-dicarboxylate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_12_3689_s_308	11371533	It is not required for the conversion of protocatechuate to pyruvate and oxaloacetate (above), and extracts of  E. coli strains carrying the  pcmF gene (on pRE1056, e.g.) did not have activity toward such substrates as 2-hydroxy-4-carboxymuconic semialdehyde and 2-pyrone-4,6-dicarboxylate.	transcription
52318	7	334951	5	NULL	NULL	0	NULL	2-pyrone-4,6-dicarboxylate	NULL		is a type of	NULL				substrate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_12_3689_s_308	11371533	It is not required for the conversion of protocatechuate to pyruvate and oxaloacetate (above), and extracts of  E. coli strains carrying the  pcmF gene (on pRE1056, e.g.) did not have activity toward such substrates as 2-hydroxy-4-carboxymuconic semialdehyde and 2-pyrone-4,6-dicarboxylate.	transcription
52319	8	334951	5	NULL	NULL	0	NULL	2-hydroxy-4-carboxymuconic semialdehyde	NULL		is a type of	NULL				substrate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_12_3689_s_308	11371533	It is not required for the conversion of protocatechuate to pyruvate and oxaloacetate (above), and extracts of  E. coli strains carrying the  pcmF gene (on pRE1056, e.g.) did not have activity toward such substrates as 2-hydroxy-4-carboxymuconic semialdehyde and 2-pyrone-4,6-dicarboxylate.	transcription
54409	1	334951	6	NULL	NULL	0	NULL	protocatechuate			is converted to					pyruvate					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_12_3689_s_308	11371533	It is not required for the conversion of protocatechuate to pyruvate and oxaloacetate (above), and extracts of  E. coli strains carrying the  pcmF gene (on pRE1056, e.g.) did not have activity toward such substrates as 2-hydroxy-4-carboxymuconic semialdehyde and 2-pyrone-4,6-dicarboxylate.	transcription
54410	2	334951	6	NULL	NULL	0	NULL	protocatechuate			is converted to					oxaloacetate					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_12_3689_s_308	11371533	It is not required for the conversion of protocatechuate to pyruvate and oxaloacetate (above), and extracts of  E. coli strains carrying the  pcmF gene (on pRE1056, e.g.) did not have activity toward such substrates as 2-hydroxy-4-carboxymuconic semialdehyde and 2-pyrone-4,6-dicarboxylate.	transcription
54411	3	334951	6	NULL	NULL	0	NULL	statement 1			occurs simultaneously with					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_12_3689_s_308	11371533	It is not required for the conversion of protocatechuate to pyruvate and oxaloacetate (above), and extracts of  E. coli strains carrying the  pcmF gene (on pRE1056, e.g.) did not have activity toward such substrates as 2-hydroxy-4-carboxymuconic semialdehyde and 2-pyrone-4,6-dicarboxylate.	transcription
52320	1	334952	5	NULL	NULL	0	NULL	OAA	NULL		is	NULL				oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_21_6679_s_126	10542169	These are the gluconeogenic conversion of oxaloacetate (OAA) to phosphoenolpyruvate (PEP) (Fig.  2G), catalyzed by the PEP carboxykinase ( 10,  11), and the conversion of malate (MAL) to pyruvate (PYR) (Fig.  2H and I) through the malic enzyme.	transcription
52321	2	334952	5	NULL	NULL	0	NULL	PEP	NULL		is	NULL				phosphoenolpyruvate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_21_6679_s_126	10542169	These are the gluconeogenic conversion of oxaloacetate (OAA) to phosphoenolpyruvate (PEP) (Fig.  2G), catalyzed by the PEP carboxykinase ( 10,  11), and the conversion of malate (MAL) to pyruvate (PYR) (Fig.  2H and I) through the malic enzyme.	transcription
52322	3	334952	5	NULL	NULL	0	NULL	MAL	NULL		is	NULL				malate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_21_6679_s_126	10542169	These are the gluconeogenic conversion of oxaloacetate (OAA) to phosphoenolpyruvate (PEP) (Fig.  2G), catalyzed by the PEP carboxykinase ( 10,  11), and the conversion of malate (MAL) to pyruvate (PYR) (Fig.  2H and I) through the malic enzyme.	transcription
52323	4	334952	5	NULL	NULL	0	NULL	PYR	NULL		is	NULL				pyruvate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_21_6679_s_126	10542169	These are the gluconeogenic conversion of oxaloacetate (OAA) to phosphoenolpyruvate (PEP) (Fig.  2G), catalyzed by the PEP carboxykinase ( 10,  11), and the conversion of malate (MAL) to pyruvate (PYR) (Fig.  2H and I) through the malic enzyme.	transcription
52324	5	334952	5	NULL	NULL	0	NULL	OAA	NULL		is converted to	NULL				PEP	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_21_6679_s_126	10542169	These are the gluconeogenic conversion of oxaloacetate (OAA) to phosphoenolpyruvate (PEP) (Fig.  2G), catalyzed by the PEP carboxykinase ( 10,  11), and the conversion of malate (MAL) to pyruvate (PYR) (Fig.  2H and I) through the malic enzyme.	transcription
52325	6	334952	5	NULL	NULL	0	NULL	PEP carboxykinase	NULL		catalyzes	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_21_6679_s_126	10542169	These are the gluconeogenic conversion of oxaloacetate (OAA) to phosphoenolpyruvate (PEP) (Fig.  2G), catalyzed by the PEP carboxykinase ( 10,  11), and the conversion of malate (MAL) to pyruvate (PYR) (Fig.  2H and I) through the malic enzyme.	transcription
52326	7	334952	5	NULL	NULL	0	NULL	MAL	NULL		is converted to	NULL				PYR	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_21_6679_s_126	10542169	These are the gluconeogenic conversion of oxaloacetate (OAA) to phosphoenolpyruvate (PEP) (Fig.  2G), catalyzed by the PEP carboxykinase ( 10,  11), and the conversion of malate (MAL) to pyruvate (PYR) (Fig.  2H and I) through the malic enzyme.	transcription
52327	8	334952	5	NULL	NULL	0	NULL	malic enzyme	NULL		catalyzes	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_21_6679_s_126	10542169	These are the gluconeogenic conversion of oxaloacetate (OAA) to phosphoenolpyruvate (PEP) (Fig.  2G), catalyzed by the PEP carboxykinase ( 10,  11), and the conversion of malate (MAL) to pyruvate (PYR) (Fig.  2H and I) through the malic enzyme.	transcription
54412	1	334952	6	NULL	NULL	0	NULL	oxaloacetate			is converted to					phosphoenolpyruvate					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_21_6679_s_126	10542169	These are the gluconeogenic conversion of oxaloacetate (OAA) to phosphoenolpyruvate (PEP) (Fig.  2G), catalyzed by the PEP carboxykinase ( 10,  11), and the conversion of malate (MAL) to pyruvate (PYR) (Fig.  2H and I) through the malic enzyme.	transcription
54413	2	334952	6	NULL	NULL	0	NULL	OAA			is					oxaloacetate					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_21_6679_s_126	10542169	These are the gluconeogenic conversion of oxaloacetate (OAA) to phosphoenolpyruvate (PEP) (Fig.  2G), catalyzed by the PEP carboxykinase ( 10,  11), and the conversion of malate (MAL) to pyruvate (PYR) (Fig.  2H and I) through the malic enzyme.	transcription
54414	3	334952	6	NULL	NULL	0	NULL	PEP			is					phosphoenolpyruvate					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_21_6679_s_126	10542169	These are the gluconeogenic conversion of oxaloacetate (OAA) to phosphoenolpyruvate (PEP) (Fig.  2G), catalyzed by the PEP carboxykinase ( 10,  11), and the conversion of malate (MAL) to pyruvate (PYR) (Fig.  2H and I) through the malic enzyme.	transcription
54415	4	334952	6	NULL	NULL	0	NULL	PEP carboxykinase			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_21_6679_s_126	10542169	These are the gluconeogenic conversion of oxaloacetate (OAA) to phosphoenolpyruvate (PEP) (Fig.  2G), catalyzed by the PEP carboxykinase ( 10,  11), and the conversion of malate (MAL) to pyruvate (PYR) (Fig.  2H and I) through the malic enzyme.	transcription
54416	5	334952	6	NULL	NULL	0	NULL	malate			is converted to					pyruvate					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_21_6679_s_126	10542169	These are the gluconeogenic conversion of oxaloacetate (OAA) to phosphoenolpyruvate (PEP) (Fig.  2G), catalyzed by the PEP carboxykinase ( 10,  11), and the conversion of malate (MAL) to pyruvate (PYR) (Fig.  2H and I) through the malic enzyme.	transcription
54417	6	334952	6	NULL	NULL	0	NULL	malic enzyme			catalyzes					statement 5					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_21_6679_s_126	10542169	These are the gluconeogenic conversion of oxaloacetate (OAA) to phosphoenolpyruvate (PEP) (Fig.  2G), catalyzed by the PEP carboxykinase ( 10,  11), and the conversion of malate (MAL) to pyruvate (PYR) (Fig.  2H and I) through the malic enzyme.	transcription
52328	1	334953	5	NULL	NULL	0	NULL	NAD(P)H	NULL		regulates	NULL	negatively			Bdh	NULL	activity of			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_3_849_s_260	9922248	Although there are several reports demonstrating that Bdh activity is negatively regulated by NAD(P)H, adenosine nucleotides, pyruvate, oxaloacetate, and 2-ketoglutarate ( 55,  71,  78), regulation of Bdh at the level of gene expression was not examined.	transcription
52329	2	334953	5	NULL	NULL	0	NULL	adenosine nucleotides	NULL		regulates	NULL	negatively			Bdh	NULL	activity of			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_3_849_s_260	9922248	Although there are several reports demonstrating that Bdh activity is negatively regulated by NAD(P)H, adenosine nucleotides, pyruvate, oxaloacetate, and 2-ketoglutarate ( 55,  71,  78), regulation of Bdh at the level of gene expression was not examined.	transcription
52330	3	334953	5	NULL	NULL	0	NULL	pyruvate	NULL		regulates	NULL	negatively			Bdh	NULL	activity of			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_3_849_s_260	9922248	Although there are several reports demonstrating that Bdh activity is negatively regulated by NAD(P)H, adenosine nucleotides, pyruvate, oxaloacetate, and 2-ketoglutarate ( 55,  71,  78), regulation of Bdh at the level of gene expression was not examined.	transcription
52331	4	334953	5	NULL	NULL	0	NULL	oxaloacetate	NULL		regulates	NULL	negatively			Bdh	NULL	activity of			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_3_849_s_260	9922248	Although there are several reports demonstrating that Bdh activity is negatively regulated by NAD(P)H, adenosine nucleotides, pyruvate, oxaloacetate, and 2-ketoglutarate ( 55,  71,  78), regulation of Bdh at the level of gene expression was not examined.	transcription
52332	5	334953	5	NULL	NULL	0	NULL	2-ketoglutarate	NULL		regulates	NULL	negatively			Bdh	NULL	activity of			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_3_849_s_260	9922248	Although there are several reports demonstrating that Bdh activity is negatively regulated by NAD(P)H, adenosine nucleotides, pyruvate, oxaloacetate, and 2-ketoglutarate ( 55,  71,  78), regulation of Bdh at the level of gene expression was not examined.	transcription
54418	1	334953	6	NULL	NULL	0	NULL	NAD(P)H			regulates		negatively			Bdh		activity of 			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_3_849_s_260	9922248	Although there are several reports demonstrating that Bdh activity is negatively regulated by NAD(P)H, adenosine nucleotides, pyruvate, oxaloacetate, and 2-ketoglutarate ( 55,  71,  78), regulation of Bdh at the level of gene expression was not examined.	transcription
54419	2	334953	6	NULL	NULL	0	NULL	adenosine nucleotides			regulates		negatively			Bdh		activity of 			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_3_849_s_260	9922248	Although there are several reports demonstrating that Bdh activity is negatively regulated by NAD(P)H, adenosine nucleotides, pyruvate, oxaloacetate, and 2-ketoglutarate ( 55,  71,  78), regulation of Bdh at the level of gene expression was not examined.	transcription
54420	3	334953	6	NULL	NULL	0	NULL	pyruvate			regulates		negatively			Bdh		activity of 			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_3_849_s_260	9922248	Although there are several reports demonstrating that Bdh activity is negatively regulated by NAD(P)H, adenosine nucleotides, pyruvate, oxaloacetate, and 2-ketoglutarate ( 55,  71,  78), regulation of Bdh at the level of gene expression was not examined.	transcription
54421	4	334953	6	NULL	NULL	0	NULL	oxaloacetate			regulates		negatively			Bdh		activity of 			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_3_849_s_260	9922248	Although there are several reports demonstrating that Bdh activity is negatively regulated by NAD(P)H, adenosine nucleotides, pyruvate, oxaloacetate, and 2-ketoglutarate ( 55,  71,  78), regulation of Bdh at the level of gene expression was not examined.	transcription
54422	5	334953	6	NULL	NULL	0	NULL	2-ketoglutarate			regulates		negatively			Bdh		activity of 			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_3_849_s_260	9922248	Although there are several reports demonstrating that Bdh activity is negatively regulated by NAD(P)H, adenosine nucleotides, pyruvate, oxaloacetate, and 2-ketoglutarate ( 55,  71,  78), regulation of Bdh at the level of gene expression was not examined.	transcription
52333	1	334954	5	NULL	NULL	0	NULL	pyruvate carboxylase	NULL	cytosolic	carboxylates	NULL				pyruvate	NULL				NULL		0	NULL	NULL	NULL	gw70_yeast_21_9_769_s_295	15282800	The mitochondrial malic enzyme, in conjunction with the cytosolic  enzymes pyruvate carboxylase, which carboxylates pyruvate producing oxaloacetate  and malate dehydrogenase, could effectively function as a futile cycle converting  NADH from cytosol at the expense of one ATP to mitochondrial NADPH, producing a transhydrogenase  effect.	transcription
52334	2	334954	5	NULL	NULL	0	NULL	statement 1	NULL		produce	NULL				oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw70_yeast_21_9_769_s_295	15282800	The mitochondrial malic enzyme, in conjunction with the cytosolic  enzymes pyruvate carboxylase, which carboxylates pyruvate producing oxaloacetate  and malate dehydrogenase, could effectively function as a futile cycle converting  NADH from cytosol at the expense of one ATP to mitochondrial NADPH, producing a transhydrogenase  effect.	transcription
52335	3	334954	5	NULL	NULL	0	NULL	malic enzyme	NULL	mitochondrial	acts in conjunction with	NULL				pyruvate carboxylase	NULL	cytosolic			NULL		0	NULL	NULL	NULL	gw70_yeast_21_9_769_s_295	15282800	The mitochondrial malic enzyme, in conjunction with the cytosolic  enzymes pyruvate carboxylase, which carboxylates pyruvate producing oxaloacetate  and malate dehydrogenase, could effectively function as a futile cycle converting  NADH from cytosol at the expense of one ATP to mitochondrial NADPH, producing a transhydrogenase  effect.	transcription
52336	4	334954	5	NULL	NULL	0	NULL	malic enzyme	NULL	mitochondrial	acts in conjunction with	NULL				malate dehydrogenase	NULL	cytosolic			NULL		0	NULL	NULL	NULL	gw70_yeast_21_9_769_s_295	15282800	The mitochondrial malic enzyme, in conjunction with the cytosolic  enzymes pyruvate carboxylase, which carboxylates pyruvate producing oxaloacetate  and malate dehydrogenase, could effectively function as a futile cycle converting  NADH from cytosol at the expense of one ATP to mitochondrial NADPH, producing a transhydrogenase  effect.	transcription
52337	5	334954	5	NULL	NULL	0	NULL	statement 3	NULL		occurs along with	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_yeast_21_9_769_s_295	15282800	The mitochondrial malic enzyme, in conjunction with the cytosolic  enzymes pyruvate carboxylase, which carboxylates pyruvate producing oxaloacetate  and malate dehydrogenase, could effectively function as a futile cycle converting  NADH from cytosol at the expense of one ATP to mitochondrial NADPH, producing a transhydrogenase  effect.	transcription
52338	6	334954	5	NULL	NULL	0	NULL	statement 5	NULL		function as	NULL	effectively			futile cycle	NULL				NULL		0	NULL	NULL	NULL	gw70_yeast_21_9_769_s_295	15282800	The mitochondrial malic enzyme, in conjunction with the cytosolic  enzymes pyruvate carboxylase, which carboxylates pyruvate producing oxaloacetate  and malate dehydrogenase, could effectively function as a futile cycle converting  NADH from cytosol at the expense of one ATP to mitochondrial NADPH, producing a transhydrogenase  effect.	transcription
52339	7	334954	5	NULL	NULL	0	NULL	NADH	NULL	cytosolic	is converted to	NULL				NADPH	NULL	mitochondrial			NULL		0	NULL	NULL	NULL	gw70_yeast_21_9_769_s_295	15282800	The mitochondrial malic enzyme, in conjunction with the cytosolic  enzymes pyruvate carboxylase, which carboxylates pyruvate producing oxaloacetate  and malate dehydrogenase, could effectively function as a futile cycle converting  NADH from cytosol at the expense of one ATP to mitochondrial NADPH, producing a transhydrogenase  effect.	transcription
52340	8	334954	5	NULL	NULL	0	NULL	statement 6	NULL		leads to	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw70_yeast_21_9_769_s_295	15282800	The mitochondrial malic enzyme, in conjunction with the cytosolic  enzymes pyruvate carboxylase, which carboxylates pyruvate producing oxaloacetate  and malate dehydrogenase, could effectively function as a futile cycle converting  NADH from cytosol at the expense of one ATP to mitochondrial NADPH, producing a transhydrogenase  effect.	transcription
52341	9	334954	5	NULL	NULL	0	NULL	statement 7	NULL		requires	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw70_yeast_21_9_769_s_295	15282800	The mitochondrial malic enzyme, in conjunction with the cytosolic  enzymes pyruvate carboxylase, which carboxylates pyruvate producing oxaloacetate  and malate dehydrogenase, could effectively function as a futile cycle converting  NADH from cytosol at the expense of one ATP to mitochondrial NADPH, producing a transhydrogenase  effect.	transcription
52342	10	334954	5	NULL	NULL	0	NULL	statement 7	NULL		produce	NULL				transhydrogenase effect	NULL				NULL		0	NULL	NULL	NULL	gw70_yeast_21_9_769_s_295	15282800	The mitochondrial malic enzyme, in conjunction with the cytosolic  enzymes pyruvate carboxylase, which carboxylates pyruvate producing oxaloacetate  and malate dehydrogenase, could effectively function as a futile cycle converting  NADH from cytosol at the expense of one ATP to mitochondrial NADPH, producing a transhydrogenase  effect.	transcription
54426	1	334954	6	NULL	NULL	0	NULL	pyruvate			is carboxylated to					oxaloacetate					NULL		0	NULL	NULL	NULL	gw70_yeast_21_9_769_s_295	15282800	The mitochondrial malic enzyme, in conjunction with the cytosolic  enzymes pyruvate carboxylase, which carboxylates pyruvate producing oxaloacetate  and malate dehydrogenase, could effectively function as a futile cycle converting  NADH from cytosol at the expense of one ATP to mitochondrial NADPH, producing a transhydrogenase  effect.	transcription
54427	2	334954	6	NULL	NULL	0	NULL	pyruvate			is carboxylated to					malate dehydrogenase					NULL		0	NULL	NULL	NULL	gw70_yeast_21_9_769_s_295	15282800	The mitochondrial malic enzyme, in conjunction with the cytosolic  enzymes pyruvate carboxylase, which carboxylates pyruvate producing oxaloacetate  and malate dehydrogenase, could effectively function as a futile cycle converting  NADH from cytosol at the expense of one ATP to mitochondrial NADPH, producing a transhydrogenase  effect.	transcription
54428	3	334954	6	NULL	NULL	0	NULL	statement 1			occurs simultaneously with					statement 2					NULL		0	NULL	NULL	NULL	gw70_yeast_21_9_769_s_295	15282800	The mitochondrial malic enzyme, in conjunction with the cytosolic  enzymes pyruvate carboxylase, which carboxylates pyruvate producing oxaloacetate  and malate dehydrogenase, could effectively function as a futile cycle converting  NADH from cytosol at the expense of one ATP to mitochondrial NADPH, producing a transhydrogenase  effect.	transcription
54442	4	334954	6	NULL	NULL	0	NULL	NADH		cytosol	is converted to					NADPH		mitochondria			NULL		0	NULL	NULL	NULL	gw70_yeast_21_9_769_s_295	15282800	The mitochondrial malic enzyme, in conjunction with the cytosolic  enzymes pyruvate carboxylase, which carboxylates pyruvate producing oxaloacetate  and malate dehydrogenase, could effectively function as a futile cycle converting  NADH from cytosol at the expense of one ATP to mitochondrial NADPH, producing a transhydrogenase  effect.	transcription
54443	5	334954	6	NULL	NULL	0	NULL	statement 4			produces					transhydrogenase effect					NULL		0	NULL	NULL	NULL	gw70_yeast_21_9_769_s_295	15282800	The mitochondrial malic enzyme, in conjunction with the cytosolic  enzymes pyruvate carboxylase, which carboxylates pyruvate producing oxaloacetate  and malate dehydrogenase, could effectively function as a futile cycle converting  NADH from cytosol at the expense of one ATP to mitochondrial NADPH, producing a transhydrogenase  effect.	transcription
52343	1	334955	5	NULL	NULL	0	NULL	PEP	NULL		is carboxylated to	NULL				oxaloacetate	NULL				NULL	R. eutropha	NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_212_2_159_s_6	12113928	In  R. eutropha three enzymes are known which mediate between the C3 and C4 compounds in the metabolism [  14 and   29]: (i) the PEP carboxykinase catalyzes the carboxylation of PEP to oxaloacetate and vice versa, (ii) the PEP synthetase catalyzes the phosphorylation of pyruvate to PEP, and (iii) the malic enzyme decarboxylates malate oxidatively to pyruvate.	transcription
52344	2	334955	5	NULL	NULL	0	NULL	oxaloacetate	NULL		is carboxylated to	NULL				PEP	NULL				NULL	R. eutropha	NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_212_2_159_s_6	12113928	In  R. eutropha three enzymes are known which mediate between the C3 and C4 compounds in the metabolism [  14 and   29]: (i) the PEP carboxykinase catalyzes the carboxylation of PEP to oxaloacetate and vice versa, (ii) the PEP synthetase catalyzes the phosphorylation of pyruvate to PEP, and (iii) the malic enzyme decarboxylates malate oxidatively to pyruvate.	transcription
52345	3	334955	5	NULL	NULL	0	NULL	PEP carboxykinase	NULL		catalyzes	NULL				statement 1	NULL				NULL	R. eutropha	0	NULL	NULL	NULL	gw60_femsmicrobiollett_212_2_159_s_6	12113928	In  R. eutropha three enzymes are known which mediate between the C3 and C4 compounds in the metabolism [  14 and   29]: (i) the PEP carboxykinase catalyzes the carboxylation of PEP to oxaloacetate and vice versa, (ii) the PEP synthetase catalyzes the phosphorylation of pyruvate to PEP, and (iii) the malic enzyme decarboxylates malate oxidatively to pyruvate.	transcription
52346	4	334955	5	NULL	NULL	0	NULL	PEP carboxykinase	NULL		catalyzes	NULL				statement 2	NULL				NULL	R. eutropha	0	NULL	NULL	NULL	gw60_femsmicrobiollett_212_2_159_s_6	12113928	In  R. eutropha three enzymes are known which mediate between the C3 and C4 compounds in the metabolism [  14 and   29]: (i) the PEP carboxykinase catalyzes the carboxylation of PEP to oxaloacetate and vice versa, (ii) the PEP synthetase catalyzes the phosphorylation of pyruvate to PEP, and (iii) the malic enzyme decarboxylates malate oxidatively to pyruvate.	transcription
52347	5	334955	5	NULL	NULL	0	NULL	pyruvate	NULL		is phosphorylated to	NULL				PEP	NULL				NULL	R. eutropha	NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_212_2_159_s_6	12113928	In  R. eutropha three enzymes are known which mediate between the C3 and C4 compounds in the metabolism [  14 and   29]: (i) the PEP carboxykinase catalyzes the carboxylation of PEP to oxaloacetate and vice versa, (ii) the PEP synthetase catalyzes the phosphorylation of pyruvate to PEP, and (iii) the malic enzyme decarboxylates malate oxidatively to pyruvate.	transcription
52348	6	334955	5	NULL	NULL	0	NULL	PEP synthetase	NULL		catalyzes	NULL				statement 5	NULL				NULL	R. eutropha	0	NULL	NULL	NULL	gw60_femsmicrobiollett_212_2_159_s_6	12113928	In  R. eutropha three enzymes are known which mediate between the C3 and C4 compounds in the metabolism [  14 and   29]: (i) the PEP carboxykinase catalyzes the carboxylation of PEP to oxaloacetate and vice versa, (ii) the PEP synthetase catalyzes the phosphorylation of pyruvate to PEP, and (iii) the malic enzyme decarboxylates malate oxidatively to pyruvate.	transcription
52349	7	334955	5	NULL	NULL	0	NULL	malate	NULL		decarboxylated to	NULL	oxidatively			pyruvate	NULL				NULL	R. eutropha	0	NULL	NULL	NULL	gw60_femsmicrobiollett_212_2_159_s_6	12113928	In  R. eutropha three enzymes are known which mediate between the C3 and C4 compounds in the metabolism [  14 and   29]: (i) the PEP carboxykinase catalyzes the carboxylation of PEP to oxaloacetate and vice versa, (ii) the PEP synthetase catalyzes the phosphorylation of pyruvate to PEP, and (iii) the malic enzyme decarboxylates malate oxidatively to pyruvate.	transcription
52350	8	334955	5	NULL	NULL	0	NULL	malic enzyme	NULL		catalyzes	NULL				statement 7	NULL				NULL	R. eutropha	NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_212_2_159_s_6	12113928	In  R. eutropha three enzymes are known which mediate between the C3 and C4 compounds in the metabolism [  14 and   29]: (i) the PEP carboxykinase catalyzes the carboxylation of PEP to oxaloacetate and vice versa, (ii) the PEP synthetase catalyzes the phosphorylation of pyruvate to PEP, and (iii) the malic enzyme decarboxylates malate oxidatively to pyruvate.	transcription
54444	1	334955	6	NULL	NULL	0	NULL	PEP			is carboxylated to					oxaloacetate					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_212_2_159_s_6	12113928	In  R. eutropha three enzymes are known which mediate between the C3 and C4 compounds in the metabolism [  14 and   29]: (i) the PEP carboxykinase catalyzes the carboxylation of PEP to oxaloacetate and vice versa, (ii) the PEP synthetase catalyzes the phosphorylation of pyruvate to PEP, and (iii) the malic enzyme decarboxylates malate oxidatively to pyruvate.	transcription
54445	2	334955	6	NULL	NULL	0	NULL	PEP carboxykinase			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_212_2_159_s_6	12113928	In  R. eutropha three enzymes are known which mediate between the C3 and C4 compounds in the metabolism [  14 and   29]: (i) the PEP carboxykinase catalyzes the carboxylation of PEP to oxaloacetate and vice versa, (ii) the PEP synthetase catalyzes the phosphorylation of pyruvate to PEP, and (iii) the malic enzyme decarboxylates malate oxidatively to pyruvate.	transcription
54446	3	334955	6	NULL	NULL	0	NULL	pyruvate			is phosphorylated to					PEP					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_212_2_159_s_6	12113928	In  R. eutropha three enzymes are known which mediate between the C3 and C4 compounds in the metabolism [  14 and   29]: (i) the PEP carboxykinase catalyzes the carboxylation of PEP to oxaloacetate and vice versa, (ii) the PEP synthetase catalyzes the phosphorylation of pyruvate to PEP, and (iii) the malic enzyme decarboxylates malate oxidatively to pyruvate.	transcription
54447	4	334955	6	NULL	NULL	0	NULL	PEP synthetase			catalyzes					statement 3					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_212_2_159_s_6	12113928	In  R. eutropha three enzymes are known which mediate between the C3 and C4 compounds in the metabolism [  14 and   29]: (i) the PEP carboxykinase catalyzes the carboxylation of PEP to oxaloacetate and vice versa, (ii) the PEP synthetase catalyzes the phosphorylation of pyruvate to PEP, and (iii) the malic enzyme decarboxylates malate oxidatively to pyruvate.	transcription
54448	5	334955	6	NULL	NULL	0	NULL	malate			decarboxylates		oxidatively			pyruvate					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_212_2_159_s_6	12113928	In  R. eutropha three enzymes are known which mediate between the C3 and C4 compounds in the metabolism [  14 and   29]: (i) the PEP carboxykinase catalyzes the carboxylation of PEP to oxaloacetate and vice versa, (ii) the PEP synthetase catalyzes the phosphorylation of pyruvate to PEP, and (iii) the malic enzyme decarboxylates malate oxidatively to pyruvate.	transcription
54449	6	334955	6	NULL	NULL	0	NULL	malic enzyme			catalyzes					statement 5					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_212_2_159_s_6	12113928	In  R. eutropha three enzymes are known which mediate between the C3 and C4 compounds in the metabolism [  14 and   29]: (i) the PEP carboxykinase catalyzes the carboxylation of PEP to oxaloacetate and vice versa, (ii) the PEP synthetase catalyzes the phosphorylation of pyruvate to PEP, and (iii) the malic enzyme decarboxylates malate oxidatively to pyruvate.	transcription
52372	1	334956	5	NULL	NULL	0	NULL	pyruvate	NULL	neuroprotective effects of;;addition of	is associated with	NULL				NAD+	NULL	normalization of;;cellular levels of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_9_3139_s_6	10777777	Favoring this indirect mechanism of GAPDH inhibition, the neuroprotective effects of pyruvate addition were associated with normalization of cellular levels of NAD+, DHAP, and FBP. Zn2+-induced neuronal death was also attenuated by addition of the energy substrate oxaloacetate, the activator of pyruvate dehydrogenase, dichloroacetate, or the inhibitors of NAD+ catabolism, niacinamide or benzamide.	transcription
52373	2	334956	5	NULL	NULL	0	NULL	pyruvate	NULL	neuroprotective effects of;;addition of	is associated with	NULL				DHAP	NULL	normalization of;;cellular levels of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_9_3139_s_6	10777777	Favoring this indirect mechanism of GAPDH inhibition, the neuroprotective effects of pyruvate addition were associated with normalization of cellular levels of NAD+, DHAP, and FBP. Zn2+-induced neuronal death was also attenuated by addition of the energy substrate oxaloacetate, the activator of pyruvate dehydrogenase, dichloroacetate, or the inhibitors of NAD+ catabolism, niacinamide or benzamide.	transcription
52374	3	334956	5	NULL	NULL	0	NULL	pyruvate	NULL	neuroprotective effects of;;addition of	is associated with	NULL				FBP	NULL	normalization of;;cellular levels of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_9_3139_s_6	10777777	Favoring this indirect mechanism of GAPDH inhibition, the neuroprotective effects of pyruvate addition were associated with normalization of cellular levels of NAD+, DHAP, and FBP. Zn2+-induced neuronal death was also attenuated by addition of the energy substrate oxaloacetate, the activator of pyruvate dehydrogenase, dichloroacetate, or the inhibitors of NAD+ catabolism, niacinamide or benzamide.	transcription
52375	4	334956	5	NULL	NULL	0	NULL	neuronal death	NULL		is induced by	NULL				Zn2+	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_20_9_3139_s_6	10777777	Favoring this indirect mechanism of GAPDH inhibition, the neuroprotective effects of pyruvate addition were associated with normalization of cellular levels of NAD+, DHAP, and FBP. Zn2+-induced neuronal death was also attenuated by addition of the energy substrate oxaloacetate, the activator of pyruvate dehydrogenase, dichloroacetate, or the inhibitors of NAD+ catabolism, niacinamide or benzamide.	transcription
52376	5	334956	5	NULL	NULL	0	NULL	oxaloacetate	NULL		is a type of	NULL				energy substrate	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_9_3139_s_6	10777777	Favoring this indirect mechanism of GAPDH inhibition, the neuroprotective effects of pyruvate addition were associated with normalization of cellular levels of NAD+, DHAP, and FBP. Zn2+-induced neuronal death was also attenuated by addition of the energy substrate oxaloacetate, the activator of pyruvate dehydrogenase, dichloroacetate, or the inhibitors of NAD+ catabolism, niacinamide or benzamide.	transcription
52377	6	334956	5	NULL	NULL	0	NULL	oxaloacetate	NULL	addition of	attenuate	NULL				statement 4	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_20_9_3139_s_6	10777777	Favoring this indirect mechanism of GAPDH inhibition, the neuroprotective effects of pyruvate addition were associated with normalization of cellular levels of NAD+, DHAP, and FBP. Zn2+-induced neuronal death was also attenuated by addition of the energy substrate oxaloacetate, the activator of pyruvate dehydrogenase, dichloroacetate, or the inhibitors of NAD+ catabolism, niacinamide or benzamide.	transcription
52378	7	334956	5	NULL	NULL	0	NULL	dichloroacetate	NULL		activates	NULL				pyruvate dehydrogenase	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_9_3139_s_6	10777777	Favoring this indirect mechanism of GAPDH inhibition, the neuroprotective effects of pyruvate addition were associated with normalization of cellular levels of NAD+, DHAP, and FBP. Zn2+-induced neuronal death was also attenuated by addition of the energy substrate oxaloacetate, the activator of pyruvate dehydrogenase, dichloroacetate, or the inhibitors of NAD+ catabolism, niacinamide or benzamide.	transcription
52379	8	334956	5	NULL	NULL	0	NULL	pyruvate dehydrogenase	NULL	addition of	attenuate	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_9_3139_s_6	10777777	Favoring this indirect mechanism of GAPDH inhibition, the neuroprotective effects of pyruvate addition were associated with normalization of cellular levels of NAD+, DHAP, and FBP. Zn2+-induced neuronal death was also attenuated by addition of the energy substrate oxaloacetate, the activator of pyruvate dehydrogenase, dichloroacetate, or the inhibitors of NAD+ catabolism, niacinamide or benzamide.	transcription
52380	9	334956	5	NULL	NULL	0	NULL	niacinamide	NULL		inhibit	NULL				NAD+	NULL	catabolism of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_9_3139_s_6	10777777	Favoring this indirect mechanism of GAPDH inhibition, the neuroprotective effects of pyruvate addition were associated with normalization of cellular levels of NAD+, DHAP, and FBP. Zn2+-induced neuronal death was also attenuated by addition of the energy substrate oxaloacetate, the activator of pyruvate dehydrogenase, dichloroacetate, or the inhibitors of NAD+ catabolism, niacinamide or benzamide.	transcription
52381	10	334956	5	NULL	NULL	0	NULL	benzamide	NULL		inhibit	NULL				NAD+	NULL	catabolism of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_9_3139_s_6	10777777	Favoring this indirect mechanism of GAPDH inhibition, the neuroprotective effects of pyruvate addition were associated with normalization of cellular levels of NAD+, DHAP, and FBP. Zn2+-induced neuronal death was also attenuated by addition of the energy substrate oxaloacetate, the activator of pyruvate dehydrogenase, dichloroacetate, or the inhibitors of NAD+ catabolism, niacinamide or benzamide.	transcription
52382	11	334956	5	NULL	NULL	0	NULL	niacinamide	NULL	addition of	attenuate	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_9_3139_s_6	10777777	Favoring this indirect mechanism of GAPDH inhibition, the neuroprotective effects of pyruvate addition were associated with normalization of cellular levels of NAD+, DHAP, and FBP. Zn2+-induced neuronal death was also attenuated by addition of the energy substrate oxaloacetate, the activator of pyruvate dehydrogenase, dichloroacetate, or the inhibitors of NAD+ catabolism, niacinamide or benzamide.	transcription
52383	12	334956	5	NULL	NULL	0	NULL	benzamide	NULL	addition of	attenuate	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_9_3139_s_6	10777777	Favoring this indirect mechanism of GAPDH inhibition, the neuroprotective effects of pyruvate addition were associated with normalization of cellular levels of NAD+, DHAP, and FBP. Zn2+-induced neuronal death was also attenuated by addition of the energy substrate oxaloacetate, the activator of pyruvate dehydrogenase, dichloroacetate, or the inhibitors of NAD+ catabolism, niacinamide or benzamide.	transcription
55279	1	334956	6	NULL	NULL	0	NULL	Zn2+			induces					neuronal death					NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_9_3139_s_6	10777777	Favoring this indirect mechanism of GAPDH inhibition, the neuroprotective effects of pyruvate addition were associated with normalization of cellular levels of NAD+, DHAP, and FBP. Zn2+-induced neuronal death was also attenuated by addition of the energy substrate oxaloacetate, the activator of pyruvate dehydrogenase, dichloroacetate, or the inhibitors of NAD+ catabolism, niacinamide or benzamide.	transcription
55280	2	334956	6	NULL	NULL	0	NULL	oxaloacetate			attenuates					statement 1					NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_9_3139_s_6	10777777	Favoring this indirect mechanism of GAPDH inhibition, the neuroprotective effects of pyruvate addition were associated with normalization of cellular levels of NAD+, DHAP, and FBP. Zn2+-induced neuronal death was also attenuated by addition of the energy substrate oxaloacetate, the activator of pyruvate dehydrogenase, dichloroacetate, or the inhibitors of NAD+ catabolism, niacinamide or benzamide.	transcription
55281	3	334956	6	NULL	NULL	0	NULL	pyruvate		addition of	effects					neuroprotection					NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_9_3139_s_6	10777777	Favoring this indirect mechanism of GAPDH inhibition, the neuroprotective effects of pyruvate addition were associated with normalization of cellular levels of NAD+, DHAP, and FBP. Zn2+-induced neuronal death was also attenuated by addition of the energy substrate oxaloacetate, the activator of pyruvate dehydrogenase, dichloroacetate, or the inhibitors of NAD+ catabolism, niacinamide or benzamide.	transcription
55282	4	334956	6	NULL	NULL	0	NULL	statement 3			is associated with					NAD+		normalization of 			NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_9_3139_s_6	10777777	Favoring this indirect mechanism of GAPDH inhibition, the neuroprotective effects of pyruvate addition were associated with normalization of cellular levels of NAD+, DHAP, and FBP. Zn2+-induced neuronal death was also attenuated by addition of the energy substrate oxaloacetate, the activator of pyruvate dehydrogenase, dichloroacetate, or the inhibitors of NAD+ catabolism, niacinamide or benzamide.	transcription
55283	5	334956	6	NULL	NULL	0	NULL	statement 3			is associated with					DHAP		normalization of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_9_3139_s_6	10777777	Favoring this indirect mechanism of GAPDH inhibition, the neuroprotective effects of pyruvate addition were associated with normalization of cellular levels of NAD+, DHAP, and FBP. Zn2+-induced neuronal death was also attenuated by addition of the energy substrate oxaloacetate, the activator of pyruvate dehydrogenase, dichloroacetate, or the inhibitors of NAD+ catabolism, niacinamide or benzamide.	transcription
55284	6	334956	6	NULL	NULL	0	NULL	statement 3			is associated with					FBP		normalization of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_9_3139_s_6	10777777	Favoring this indirect mechanism of GAPDH inhibition, the neuroprotective effects of pyruvate addition were associated with normalization of cellular levels of NAD+, DHAP, and FBP. Zn2+-induced neuronal death was also attenuated by addition of the energy substrate oxaloacetate, the activator of pyruvate dehydrogenase, dichloroacetate, or the inhibitors of NAD+ catabolism, niacinamide or benzamide.	transcription
52351	1	334957	5	NULL	NULL	0	NULL	PEP	NULL		is synthesized from	NULL				oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_17_6231_s_8	16109965	The PckA route is a one-step reaction in which PEP is synthesized from oxaloacetate catalyzed by PckA, and the malic enzyme-PpsA (or PPDK) route consists of two reactions: the first reaction is the conversion of malate to pyruvate catalyzed by the malic enzyme MaeA or MaeB and the second reaction is the synthesis of PEP from pyruvate catalyzed by PpsA using pyruvate, H2O, and ATP as substrates or by PPDK using pyruvate, phosphate, and ATP as substrates ( ,  ).	transcription
52352	2	334957	5	NULL	NULL	0	NULL	PckA	NULL		catalyzes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_17_6231_s_8	16109965	The PckA route is a one-step reaction in which PEP is synthesized from oxaloacetate catalyzed by PckA, and the malic enzyme-PpsA (or PPDK) route consists of two reactions: the first reaction is the conversion of malate to pyruvate catalyzed by the malic enzyme MaeA or MaeB and the second reaction is the synthesis of PEP from pyruvate catalyzed by PpsA using pyruvate, H2O, and ATP as substrates or by PPDK using pyruvate, phosphate, and ATP as substrates ( ,  ).	transcription
52353	3	334957	5	NULL	NULL	0	NULL	statement 1	NULL		refers to	NULL				PckA route	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_17_6231_s_8	16109965	The PckA route is a one-step reaction in which PEP is synthesized from oxaloacetate catalyzed by PckA, and the malic enzyme-PpsA (or PPDK) route consists of two reactions: the first reaction is the conversion of malate to pyruvate catalyzed by the malic enzyme MaeA or MaeB and the second reaction is the synthesis of PEP from pyruvate catalyzed by PpsA using pyruvate, H2O, and ATP as substrates or by PPDK using pyruvate, phosphate, and ATP as substrates ( ,  ).	transcription
52354	4	334957	5	NULL	NULL	0	NULL	malate	NULL		is converted to	NULL				pyruvate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_17_6231_s_8	16109965	The PckA route is a one-step reaction in which PEP is synthesized from oxaloacetate catalyzed by PckA, and the malic enzyme-PpsA (or PPDK) route consists of two reactions: the first reaction is the conversion of malate to pyruvate catalyzed by the malic enzyme MaeA or MaeB and the second reaction is the synthesis of PEP from pyruvate catalyzed by PpsA using pyruvate, H2O, and ATP as substrates or by PPDK using pyruvate, phosphate, and ATP as substrates ( ,  ).	transcription
52355	5	334957	5	NULL	NULL	0	NULL	MaeA	NULL		catalyzes	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_17_6231_s_8	16109965	The PckA route is a one-step reaction in which PEP is synthesized from oxaloacetate catalyzed by PckA, and the malic enzyme-PpsA (or PPDK) route consists of two reactions: the first reaction is the conversion of malate to pyruvate catalyzed by the malic enzyme MaeA or MaeB and the second reaction is the synthesis of PEP from pyruvate catalyzed by PpsA using pyruvate, H2O, and ATP as substrates or by PPDK using pyruvate, phosphate, and ATP as substrates ( ,  ).	transcription
52356	6	334957	5	NULL	NULL	0	NULL	MaeB	NULL		catalyzes	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_17_6231_s_8	16109965	The PckA route is a one-step reaction in which PEP is synthesized from oxaloacetate catalyzed by PckA, and the malic enzyme-PpsA (or PPDK) route consists of two reactions: the first reaction is the conversion of malate to pyruvate catalyzed by the malic enzyme MaeA or MaeB and the second reaction is the synthesis of PEP from pyruvate catalyzed by PpsA using pyruvate, H2O, and ATP as substrates or by PPDK using pyruvate, phosphate, and ATP as substrates ( ,  ).	transcription
52357	7	334957	5	NULL	NULL	0	NULL	statement 5	NULL		is an alternative to	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_17_6231_s_8	16109965	The PckA route is a one-step reaction in which PEP is synthesized from oxaloacetate catalyzed by PckA, and the malic enzyme-PpsA (or PPDK) route consists of two reactions: the first reaction is the conversion of malate to pyruvate catalyzed by the malic enzyme MaeA or MaeB and the second reaction is the synthesis of PEP from pyruvate catalyzed by PpsA using pyruvate, H2O, and ATP as substrates or by PPDK using pyruvate, phosphate, and ATP as substrates ( ,  ).	transcription
52358	8	334957	5	NULL	NULL	0	NULL	MaeA	NULL		is a type of	NULL				malic enzyme	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_17_6231_s_8	16109965	The PckA route is a one-step reaction in which PEP is synthesized from oxaloacetate catalyzed by PckA, and the malic enzyme-PpsA (or PPDK) route consists of two reactions: the first reaction is the conversion of malate to pyruvate catalyzed by the malic enzyme MaeA or MaeB and the second reaction is the synthesis of PEP from pyruvate catalyzed by PpsA using pyruvate, H2O, and ATP as substrates or by PPDK using pyruvate, phosphate, and ATP as substrates ( ,  ).	transcription
52359	9	334957	5	NULL	NULL	0	NULL	MaeB	NULL		is a type of	NULL				malic enzyme	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_17_6231_s_8	16109965	The PckA route is a one-step reaction in which PEP is synthesized from oxaloacetate catalyzed by PckA, and the malic enzyme-PpsA (or PPDK) route consists of two reactions: the first reaction is the conversion of malate to pyruvate catalyzed by the malic enzyme MaeA or MaeB and the second reaction is the synthesis of PEP from pyruvate catalyzed by PpsA using pyruvate, H2O, and ATP as substrates or by PPDK using pyruvate, phosphate, and ATP as substrates ( ,  ).	transcription
52360	10	334957	5	NULL	NULL	0	NULL	PEP	NULL		is synthesized from	NULL				pyruvate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_17_6231_s_8	16109965	The PckA route is a one-step reaction in which PEP is synthesized from oxaloacetate catalyzed by PckA, and the malic enzyme-PpsA (or PPDK) route consists of two reactions: the first reaction is the conversion of malate to pyruvate catalyzed by the malic enzyme MaeA or MaeB and the second reaction is the synthesis of PEP from pyruvate catalyzed by PpsA using pyruvate, H2O, and ATP as substrates or by PPDK using pyruvate, phosphate, and ATP as substrates ( ,  ).	transcription
52361	11	334957	5	NULL	NULL	0	NULL	PpsA	NULL		catalyzes	NULL				statement 10	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_17_6231_s_8	16109965	The PckA route is a one-step reaction in which PEP is synthesized from oxaloacetate catalyzed by PckA, and the malic enzyme-PpsA (or PPDK) route consists of two reactions: the first reaction is the conversion of malate to pyruvate catalyzed by the malic enzyme MaeA or MaeB and the second reaction is the synthesis of PEP from pyruvate catalyzed by PpsA using pyruvate, H2O, and ATP as substrates or by PPDK using pyruvate, phosphate, and ATP as substrates ( ,  ).	transcription
52362	12	334957	5	NULL	NULL	0	NULL	pyruvate	NULL		is a substrate for	NULL				PpsA	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_17_6231_s_8	16109965	The PckA route is a one-step reaction in which PEP is synthesized from oxaloacetate catalyzed by PckA, and the malic enzyme-PpsA (or PPDK) route consists of two reactions: the first reaction is the conversion of malate to pyruvate catalyzed by the malic enzyme MaeA or MaeB and the second reaction is the synthesis of PEP from pyruvate catalyzed by PpsA using pyruvate, H2O, and ATP as substrates or by PPDK using pyruvate, phosphate, and ATP as substrates ( ,  ).	transcription
52363	13	334957	5	NULL	NULL	0	NULL	H2O	NULL		is a substrate for	NULL				PpsA	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_17_6231_s_8	16109965	The PckA route is a one-step reaction in which PEP is synthesized from oxaloacetate catalyzed by PckA, and the malic enzyme-PpsA (or PPDK) route consists of two reactions: the first reaction is the conversion of malate to pyruvate catalyzed by the malic enzyme MaeA or MaeB and the second reaction is the synthesis of PEP from pyruvate catalyzed by PpsA using pyruvate, H2O, and ATP as substrates or by PPDK using pyruvate, phosphate, and ATP as substrates ( ,  ).	transcription
52364	14	334957	5	NULL	NULL	0	NULL	ATP	NULL		is a substrate for	NULL				PpsA	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_17_6231_s_8	16109965	The PckA route is a one-step reaction in which PEP is synthesized from oxaloacetate catalyzed by PckA, and the malic enzyme-PpsA (or PPDK) route consists of two reactions: the first reaction is the conversion of malate to pyruvate catalyzed by the malic enzyme MaeA or MaeB and the second reaction is the synthesis of PEP from pyruvate catalyzed by PpsA using pyruvate, H2O, and ATP as substrates or by PPDK using pyruvate, phosphate, and ATP as substrates ( ,  ).	transcription
52365	15	334957	5	NULL	NULL	0	NULL	PPDK	NULL		catalyzes	NULL				statement 10	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_17_6231_s_8	16109965	The PckA route is a one-step reaction in which PEP is synthesized from oxaloacetate catalyzed by PckA, and the malic enzyme-PpsA (or PPDK) route consists of two reactions: the first reaction is the conversion of malate to pyruvate catalyzed by the malic enzyme MaeA or MaeB and the second reaction is the synthesis of PEP from pyruvate catalyzed by PpsA using pyruvate, H2O, and ATP as substrates or by PPDK using pyruvate, phosphate, and ATP as substrates ( ,  ).	transcription
52366	16	334957	5	NULL	NULL	0	NULL	pyruvate	NULL		is a substrate for	NULL				PPDK	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_17_6231_s_8	16109965	The PckA route is a one-step reaction in which PEP is synthesized from oxaloacetate catalyzed by PckA, and the malic enzyme-PpsA (or PPDK) route consists of two reactions: the first reaction is the conversion of malate to pyruvate catalyzed by the malic enzyme MaeA or MaeB and the second reaction is the synthesis of PEP from pyruvate catalyzed by PpsA using pyruvate, H2O, and ATP as substrates or by PPDK using pyruvate, phosphate, and ATP as substrates ( ,  ).	transcription
52367	17	334957	5	NULL	NULL	0	NULL	phosphate	NULL		is a substrate for	NULL				PPDK	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_17_6231_s_8	16109965	The PckA route is a one-step reaction in which PEP is synthesized from oxaloacetate catalyzed by PckA, and the malic enzyme-PpsA (or PPDK) route consists of two reactions: the first reaction is the conversion of malate to pyruvate catalyzed by the malic enzyme MaeA or MaeB and the second reaction is the synthesis of PEP from pyruvate catalyzed by PpsA using pyruvate, H2O, and ATP as substrates or by PPDK using pyruvate, phosphate, and ATP as substrates ( ,  ).	transcription
52368	18	334957	5	NULL	NULL	0	NULL	ATP	NULL		is a substrate for	NULL				PPDK	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_17_6231_s_8	16109965	The PckA route is a one-step reaction in which PEP is synthesized from oxaloacetate catalyzed by PckA, and the malic enzyme-PpsA (or PPDK) route consists of two reactions: the first reaction is the conversion of malate to pyruvate catalyzed by the malic enzyme MaeA or MaeB and the second reaction is the synthesis of PEP from pyruvate catalyzed by PpsA using pyruvate, H2O, and ATP as substrates or by PPDK using pyruvate, phosphate, and ATP as substrates ( ,  ).	transcription
52369	19	334957	5	NULL	NULL	0	NULL	statement 11	NULL		is an alternative to	NULL				statement 15	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_187_17_6231_s_8	16109965	The PckA route is a one-step reaction in which PEP is synthesized from oxaloacetate catalyzed by PckA, and the malic enzyme-PpsA (or PPDK) route consists of two reactions: the first reaction is the conversion of malate to pyruvate catalyzed by the malic enzyme MaeA or MaeB and the second reaction is the synthesis of PEP from pyruvate catalyzed by PpsA using pyruvate, H2O, and ATP as substrates or by PPDK using pyruvate, phosphate, and ATP as substrates ( ,  ).	transcription
52370	20	334957	5	NULL	NULL	0	NULL	statement 7	NULL		occurs simultaneously with	NULL				statement 19	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_17_6231_s_8	16109965	The PckA route is a one-step reaction in which PEP is synthesized from oxaloacetate catalyzed by PckA, and the malic enzyme-PpsA (or PPDK) route consists of two reactions: the first reaction is the conversion of malate to pyruvate catalyzed by the malic enzyme MaeA or MaeB and the second reaction is the synthesis of PEP from pyruvate catalyzed by PpsA using pyruvate, H2O, and ATP as substrates or by PPDK using pyruvate, phosphate, and ATP as substrates ( ,  ).	transcription
52371	21	334957	5	NULL	NULL	0	NULL	statement 20	NULL		refers to	NULL				malic enzyme-PpsA (or PPDK) route	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_17_6231_s_8	16109965	The PckA route is a one-step reaction in which PEP is synthesized from oxaloacetate catalyzed by PckA, and the malic enzyme-PpsA (or PPDK) route consists of two reactions: the first reaction is the conversion of malate to pyruvate catalyzed by the malic enzyme MaeA or MaeB and the second reaction is the synthesis of PEP from pyruvate catalyzed by PpsA using pyruvate, H2O, and ATP as substrates or by PPDK using pyruvate, phosphate, and ATP as substrates ( ,  ).	transcription
55286	1	334957	6	NULL	NULL	0	NULL	oxaloacetate			synthesizes					PEP					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_17_6231_s_8	16109965	The PckA route is a one-step reaction in which PEP is synthesized from oxaloacetate catalyzed by PckA, and the malic enzyme-PpsA (or PPDK) route consists of two reactions: the first reaction is the conversion of malate to pyruvate catalyzed by the malic enzyme MaeA or MaeB and the second reaction is the synthesis of PEP from pyruvate catalyzed by PpsA using pyruvate, H2O, and ATP as substrates or by PPDK using pyruvate, phosphate, and ATP as substrates ( ,  ).	transcription
55287	2	334957	6	NULL	NULL	0	NULL	PckA			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_17_6231_s_8	16109965	The PckA route is a one-step reaction in which PEP is synthesized from oxaloacetate catalyzed by PckA, and the malic enzyme-PpsA (or PPDK) route consists of two reactions: the first reaction is the conversion of malate to pyruvate catalyzed by the malic enzyme MaeA or MaeB and the second reaction is the synthesis of PEP from pyruvate catalyzed by PpsA using pyruvate, H2O, and ATP as substrates or by PPDK using pyruvate, phosphate, and ATP as substrates ( ,  ).	transcription
55288	3	334957	6	NULL	NULL	0	NULL	malate			is converted to					pyruvate					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_17_6231_s_8	16109965	The PckA route is a one-step reaction in which PEP is synthesized from oxaloacetate catalyzed by PckA, and the malic enzyme-PpsA (or PPDK) route consists of two reactions: the first reaction is the conversion of malate to pyruvate catalyzed by the malic enzyme MaeA or MaeB and the second reaction is the synthesis of PEP from pyruvate catalyzed by PpsA using pyruvate, H2O, and ATP as substrates or by PPDK using pyruvate, phosphate, and ATP as substrates ( ,  ).	transcription
55289	4	334957	6	NULL	NULL	0	NULL	MaeA			catalyzes					statement 3					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_17_6231_s_8	16109965	The PckA route is a one-step reaction in which PEP is synthesized from oxaloacetate catalyzed by PckA, and the malic enzyme-PpsA (or PPDK) route consists of two reactions: the first reaction is the conversion of malate to pyruvate catalyzed by the malic enzyme MaeA or MaeB and the second reaction is the synthesis of PEP from pyruvate catalyzed by PpsA using pyruvate, H2O, and ATP as substrates or by PPDK using pyruvate, phosphate, and ATP as substrates ( ,  ).	transcription
55290	5	334957	6	NULL	NULL	0	NULL	MaeB			catalyzes					statement 3					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_17_6231_s_8	16109965	The PckA route is a one-step reaction in which PEP is synthesized from oxaloacetate catalyzed by PckA, and the malic enzyme-PpsA (or PPDK) route consists of two reactions: the first reaction is the conversion of malate to pyruvate catalyzed by the malic enzyme MaeA or MaeB and the second reaction is the synthesis of PEP from pyruvate catalyzed by PpsA using pyruvate, H2O, and ATP as substrates or by PPDK using pyruvate, phosphate, and ATP as substrates ( ,  ).	transcription
55291	6	334957	6	NULL	NULL	0	NULL	pyruvate			synthesizes					PEP					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_17_6231_s_8	16109965	The PckA route is a one-step reaction in which PEP is synthesized from oxaloacetate catalyzed by PckA, and the malic enzyme-PpsA (or PPDK) route consists of two reactions: the first reaction is the conversion of malate to pyruvate catalyzed by the malic enzyme MaeA or MaeB and the second reaction is the synthesis of PEP from pyruvate catalyzed by PpsA using pyruvate, H2O, and ATP as substrates or by PPDK using pyruvate, phosphate, and ATP as substrates ( ,  ).	transcription
55292	7	334957	6	NULL	NULL	0	NULL	PpsA			catalyzes					statement 6					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_17_6231_s_8	16109965	The PckA route is a one-step reaction in which PEP is synthesized from oxaloacetate catalyzed by PckA, and the malic enzyme-PpsA (or PPDK) route consists of two reactions: the first reaction is the conversion of malate to pyruvate catalyzed by the malic enzyme MaeA or MaeB and the second reaction is the synthesis of PEP from pyruvate catalyzed by PpsA using pyruvate, H2O, and ATP as substrates or by PPDK using pyruvate, phosphate, and ATP as substrates ( ,  ).	transcription
55293	8	334957	6	NULL	NULL	0	NULL	PPDK			catalyzes					statement 6					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_17_6231_s_8	16109965	The PckA route is a one-step reaction in which PEP is synthesized from oxaloacetate catalyzed by PckA, and the malic enzyme-PpsA (or PPDK) route consists of two reactions: the first reaction is the conversion of malate to pyruvate catalyzed by the malic enzyme MaeA or MaeB and the second reaction is the synthesis of PEP from pyruvate catalyzed by PpsA using pyruvate, H2O, and ATP as substrates or by PPDK using pyruvate, phosphate, and ATP as substrates ( ,  ).	transcription
52384	1	334958	5	NULL	NULL	0	NULL	pyruvate	NULL	carboxylation of	is necessary for	NULL				oxygen	NULL	maximal consumption of			NULL	hamster brown adipose tissue	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_29_27466_s_29	15917242	Pyruvate carboxylation was shown to be necessary in hamster brown adipose tissue for maximal oxygen consumption in norepinephrine-stimulated respiration, even when drainage of the citric acid cycle for amino acid synthesis is eliminated, suggesting that the provision of oxaloacetate promotes the oxidation of acetyl-CoA from fatty acid degradation ( ,  ).	transcription
52385	2	334958	5	NULL	NULL	0	NULL	statement 1	NULL		occurs in	NULL				respiration	NULL	norepinephrine-stimulated			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_27466_s_29	15917242	Pyruvate carboxylation was shown to be necessary in hamster brown adipose tissue for maximal oxygen consumption in norepinephrine-stimulated respiration, even when drainage of the citric acid cycle for amino acid synthesis is eliminated, suggesting that the provision of oxaloacetate promotes the oxidation of acetyl-CoA from fatty acid degradation ( ,  ).	transcription
52386	3	334958	5	NULL	NULL	0	NULL	acetyl-CoA	NULL	oxidation of	is promoted from	NULL				fatty acid	NULL	degradation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_27466_s_29	15917242	Pyruvate carboxylation was shown to be necessary in hamster brown adipose tissue for maximal oxygen consumption in norepinephrine-stimulated respiration, even when drainage of the citric acid cycle for amino acid synthesis is eliminated, suggesting that the provision of oxaloacetate promotes the oxidation of acetyl-CoA from fatty acid degradation ( ,  ).	transcription
52387	4	334958	5	NULL	NULL	0	NULL	oxaloacetate	NULL		performs	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_27466_s_29	15917242	Pyruvate carboxylation was shown to be necessary in hamster brown adipose tissue for maximal oxygen consumption in norepinephrine-stimulated respiration, even when drainage of the citric acid cycle for amino acid synthesis is eliminated, suggesting that the provision of oxaloacetate promotes the oxidation of acetyl-CoA from fatty acid degradation ( ,  ).	transcription
55302	1	334958	6	NULL	NULL	0	NULL	pyruvate		carboxylation of 	is necessary in					brown adipose tissue		hamster			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_27466_s_29	15917242	Pyruvate carboxylation was shown to be necessary in hamster brown adipose tissue for maximal oxygen consumption in norepinephrine-stimulated respiration, even when drainage of the citric acid cycle for amino acid synthesis is eliminated, suggesting that the provision of oxaloacetate promotes the oxidation of acetyl-CoA from fatty acid degradation ( ,  ).	transcription
55303	2	334958	6	NULL	NULL	0	NULL	norepinephrine			stimulates					respiration					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_27466_s_29	15917242	Pyruvate carboxylation was shown to be necessary in hamster brown adipose tissue for maximal oxygen consumption in norepinephrine-stimulated respiration, even when drainage of the citric acid cycle for amino acid synthesis is eliminated, suggesting that the provision of oxaloacetate promotes the oxidation of acetyl-CoA from fatty acid degradation ( ,  ).	transcription
55306	3	334958	6	NULL	NULL	0	NULL	statement 1			is required for					oxygen		consumption of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_27466_s_29	15917242	Pyruvate carboxylation was shown to be necessary in hamster brown adipose tissue for maximal oxygen consumption in norepinephrine-stimulated respiration, even when drainage of the citric acid cycle for amino acid synthesis is eliminated, suggesting that the provision of oxaloacetate promotes the oxidation of acetyl-CoA from fatty acid degradation ( ,  ).	transcription
55309	4	334958	6	NULL	NULL	0	NULL	oxaloacetate			promotes					acetyl-CoA		oxidation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_27466_s_29	15917242	Pyruvate carboxylation was shown to be necessary in hamster brown adipose tissue for maximal oxygen consumption in norepinephrine-stimulated respiration, even when drainage of the citric acid cycle for amino acid synthesis is eliminated, suggesting that the provision of oxaloacetate promotes the oxidation of acetyl-CoA from fatty acid degradation ( ,  ).	transcription
55311	5	334958	6	NULL	NULL	0	NULL	statement 4			occurs during					fatty acid		degradation of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_27466_s_29	15917242	Pyruvate carboxylation was shown to be necessary in hamster brown adipose tissue for maximal oxygen consumption in norepinephrine-stimulated respiration, even when drainage of the citric acid cycle for amino acid synthesis is eliminated, suggesting that the provision of oxaloacetate promotes the oxidation of acetyl-CoA from fatty acid degradation ( ,  ).	transcription
52388	1	334959	5	NULL	NULL	0	NULL	mitochondria	NULL		respires on	NULL				pyruvate & malate	NULL				NULL		0	NULL	NULL	NULL	gw70_jneurosci_23_12_4858_s_122	12832508	These measurements were similar  between the two tissue types whether the mitochondria were respiring on the  complex I substrates, pyruvate plus malate, or the complex II substrate,  succinate (plus glutamate to remove oxaloacetate, an inhibitor of succinate  dehydrogenase, by transamination)  (Lehninger et al., 1993 ).	transcription
52389	2	334959	5	NULL	NULL	0	NULL	pyruvate & malate	NULL		is a type of	NULL				complex I substrate	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jneurosci_23_12_4858_s_122	12832508	These measurements were similar  between the two tissue types whether the mitochondria were respiring on the  complex I substrates, pyruvate plus malate, or the complex II substrate,  succinate (plus glutamate to remove oxaloacetate, an inhibitor of succinate  dehydrogenase, by transamination)  (Lehninger et al., 1993 ).	transcription
52390	3	334959	5	NULL	NULL	0	NULL	mitochondria	NULL		respires on	NULL				succinate & glutamate	NULL				NULL		0	NULL	NULL	NULL	gw70_jneurosci_23_12_4858_s_122	12832508	These measurements were similar  between the two tissue types whether the mitochondria were respiring on the  complex I substrates, pyruvate plus malate, or the complex II substrate,  succinate (plus glutamate to remove oxaloacetate, an inhibitor of succinate  dehydrogenase, by transamination)  (Lehninger et al., 1993 ).	transcription
52391	4	334959	5	NULL	NULL	0	NULL	succinate	NULL		is a type of	NULL				complex II substrate	NULL				NULL		0	NULL	NULL	NULL	gw70_jneurosci_23_12_4858_s_122	12832508	These measurements were similar  between the two tissue types whether the mitochondria were respiring on the  complex I substrates, pyruvate plus malate, or the complex II substrate,  succinate (plus glutamate to remove oxaloacetate, an inhibitor of succinate  dehydrogenase, by transamination)  (Lehninger et al., 1993 ).	transcription
52392	5	334959	5	NULL	NULL	0	NULL	statement 3	NULL		removes	NULL				oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw70_jneurosci_23_12_4858_s_122	12832508	These measurements were similar  between the two tissue types whether the mitochondria were respiring on the  complex I substrates, pyruvate plus malate, or the complex II substrate,  succinate (plus glutamate to remove oxaloacetate, an inhibitor of succinate  dehydrogenase, by transamination)  (Lehninger et al., 1993 ).	transcription
52393	6	334959	5	NULL	NULL	0	NULL	oxaloacetate	NULL		is an inhibitor of	NULL				succinate dehydrogenase	NULL				NULL		0	NULL	NULL	NULL	gw70_jneurosci_23_12_4858_s_122	12832508	These measurements were similar  between the two tissue types whether the mitochondria were respiring on the  complex I substrates, pyruvate plus malate, or the complex II substrate,  succinate (plus glutamate to remove oxaloacetate, an inhibitor of succinate  dehydrogenase, by transamination)  (Lehninger et al., 1993 ).	transcription
52394	7	334959	5	NULL	NULL	0	NULL	transamination	NULL		causes	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw70_jneurosci_23_12_4858_s_122	12832508	These measurements were similar  between the two tissue types whether the mitochondria were respiring on the  complex I substrates, pyruvate plus malate, or the complex II substrate,  succinate (plus glutamate to remove oxaloacetate, an inhibitor of succinate  dehydrogenase, by transamination)  (Lehninger et al., 1993 ).	transcription
52395	1	334960	5	NULL	NULL	0	NULL	E. coli	NULL		does not possess	NULL				pyruvate carboxylase	NULL				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_24_6892_s_273	11092847	Since  E. coli does not possess a pyruvate carboxylase and assuming, as seems to be the case in  C. glutamicum, that MQO catalyzes malate oxidation while MDH reduces oxaloacetate, the absence of a phenotype for the  mqo deletion mutant in  E. coli might be due to a PEP shunt taking over its function (Fig.  4).	transcription
52396	2	334960	5	NULL	NULL	0	NULL	MQO	NULL		catalyzes	NULL				malate	NULL	oxidation of			NULL	C. glutamicum	0	NULL	NULL	NULL	gw60_jbacteriol_182_24_6892_s_273	11092847	Since  E. coli does not possess a pyruvate carboxylase and assuming, as seems to be the case in  C. glutamicum, that MQO catalyzes malate oxidation while MDH reduces oxaloacetate, the absence of a phenotype for the  mqo deletion mutant in  E. coli might be due to a PEP shunt taking over its function (Fig.  4).	transcription
52397	3	334960	5	NULL	NULL	0	NULL	MDH	NULL		reduces	NULL				oxaloacetate	NULL				NULL	C. glutamicum	0	NULL	NULL	NULL	gw60_jbacteriol_182_24_6892_s_273	11092847	Since  E. coli does not possess a pyruvate carboxylase and assuming, as seems to be the case in  C. glutamicum, that MQO catalyzes malate oxidation while MDH reduces oxaloacetate, the absence of a phenotype for the  mqo deletion mutant in  E. coli might be due to a PEP shunt taking over its function (Fig.  4).	transcription
55320	1	334960	6	NULL	NULL	0	NULL	MQO			catalyzes					malate		oxidation of			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_24_6892_s_273	11092847	Since  E. coli does not possess a pyruvate carboxylase and assuming, as seems to be the case in  C. glutamicum, that MQO catalyzes malate oxidation while MDH reduces oxaloacetate, the absence of a phenotype for the  mqo deletion mutant in  E. coli might be due to a PEP shunt taking over its function (Fig.  4).	transcription
55322	2	334960	6	NULL	NULL	0	NULL	MDH			reduces					oxaloacetate					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_182_24_6892_s_273	11092847	Since  E. coli does not possess a pyruvate carboxylase and assuming, as seems to be the case in  C. glutamicum, that MQO catalyzes malate oxidation while MDH reduces oxaloacetate, the absence of a phenotype for the  mqo deletion mutant in  E. coli might be due to a PEP shunt taking over its function (Fig.  4).	transcription
52398	1	334961	5	NULL	NULL	0	NULL	ADP1	NULL	Acinetobacter sp. strain 	lacks	NULL				pyruvate kinase	NULL	gene encoding			NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_2_1410_s_162	16461694	Since CGP biosynthesis in cells of  Acinetobacter sp. strain ADP1 using sugars or other carbohydrates as substrates gave only low amounts of CGP and since it was recently reported that  Acinetobacter sp. strain ADP1 is lacking a gene encoding pyruvate kinase, which is involved in the conversion of carbohydrates to pyruvate ( ), the phosphoenolpyruvate carboxylase encoded by  pepC catalyzing the conversion of phosphoenolpyruvate to oxaloacetate as one of the anaplerotic reactions was also overexpressed to augment the utilization of carbohydrates and to ultimately increase the metabolic flux towards 2-oxoglutarate, which is the substrate for glutamate and subsequently arginine biosynthesis.	transcription
52399	2	334961	5	NULL	NULL	0	NULL	carbohydrates	NULL		is converted to	NULL				pyruvate	NULL				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_2_1410_s_162	16461694	Since CGP biosynthesis in cells of  Acinetobacter sp. strain ADP1 using sugars or other carbohydrates as substrates gave only low amounts of CGP and since it was recently reported that  Acinetobacter sp. strain ADP1 is lacking a gene encoding pyruvate kinase, which is involved in the conversion of carbohydrates to pyruvate ( ), the phosphoenolpyruvate carboxylase encoded by  pepC catalyzing the conversion of phosphoenolpyruvate to oxaloacetate as one of the anaplerotic reactions was also overexpressed to augment the utilization of carbohydrates and to ultimately increase the metabolic flux towards 2-oxoglutarate, which is the substrate for glutamate and subsequently arginine biosynthesis.	transcription
52400	3	334961	5	NULL	NULL	0	NULL	pyruvate kinase	NULL		is involved in	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_2_1410_s_162	16461694	Since CGP biosynthesis in cells of  Acinetobacter sp. strain ADP1 using sugars or other carbohydrates as substrates gave only low amounts of CGP and since it was recently reported that  Acinetobacter sp. strain ADP1 is lacking a gene encoding pyruvate kinase, which is involved in the conversion of carbohydrates to pyruvate ( ), the phosphoenolpyruvate carboxylase encoded by  pepC catalyzing the conversion of phosphoenolpyruvate to oxaloacetate as one of the anaplerotic reactions was also overexpressed to augment the utilization of carbohydrates and to ultimately increase the metabolic flux towards 2-oxoglutarate, which is the substrate for glutamate and subsequently arginine biosynthesis.	transcription
52401	4	334961	5	NULL	NULL	0	NULL	phosphoenolpyruvate carboxylase	NULL		is encoded by	NULL				pepC	NULL				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_2_1410_s_162	16461694	Since CGP biosynthesis in cells of  Acinetobacter sp. strain ADP1 using sugars or other carbohydrates as substrates gave only low amounts of CGP and since it was recently reported that  Acinetobacter sp. strain ADP1 is lacking a gene encoding pyruvate kinase, which is involved in the conversion of carbohydrates to pyruvate ( ), the phosphoenolpyruvate carboxylase encoded by  pepC catalyzing the conversion of phosphoenolpyruvate to oxaloacetate as one of the anaplerotic reactions was also overexpressed to augment the utilization of carbohydrates and to ultimately increase the metabolic flux towards 2-oxoglutarate, which is the substrate for glutamate and subsequently arginine biosynthesis.	transcription
52402	5	334961	5	NULL	NULL	0	NULL	phosphoenolpyruvate	NULL		is converted to	NULL				oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_2_1410_s_162	16461694	Since CGP biosynthesis in cells of  Acinetobacter sp. strain ADP1 using sugars or other carbohydrates as substrates gave only low amounts of CGP and since it was recently reported that  Acinetobacter sp. strain ADP1 is lacking a gene encoding pyruvate kinase, which is involved in the conversion of carbohydrates to pyruvate ( ), the phosphoenolpyruvate carboxylase encoded by  pepC catalyzing the conversion of phosphoenolpyruvate to oxaloacetate as one of the anaplerotic reactions was also overexpressed to augment the utilization of carbohydrates and to ultimately increase the metabolic flux towards 2-oxoglutarate, which is the substrate for glutamate and subsequently arginine biosynthesis.	transcription
52403	6	334961	5	NULL	NULL	0	NULL	pepC	NULL		catalyzes	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_2_1410_s_162	16461694	Since CGP biosynthesis in cells of  Acinetobacter sp. strain ADP1 using sugars or other carbohydrates as substrates gave only low amounts of CGP and since it was recently reported that  Acinetobacter sp. strain ADP1 is lacking a gene encoding pyruvate kinase, which is involved in the conversion of carbohydrates to pyruvate ( ), the phosphoenolpyruvate carboxylase encoded by  pepC catalyzing the conversion of phosphoenolpyruvate to oxaloacetate as one of the anaplerotic reactions was also overexpressed to augment the utilization of carbohydrates and to ultimately increase the metabolic flux towards 2-oxoglutarate, which is the substrate for glutamate and subsequently arginine biosynthesis.	transcription
52404	7	334961	5	NULL	NULL	0	NULL	statement 6	NULL		is a type of	NULL				anaplerotic reactions	NULL				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_2_1410_s_162	16461694	Since CGP biosynthesis in cells of  Acinetobacter sp. strain ADP1 using sugars or other carbohydrates as substrates gave only low amounts of CGP and since it was recently reported that  Acinetobacter sp. strain ADP1 is lacking a gene encoding pyruvate kinase, which is involved in the conversion of carbohydrates to pyruvate ( ), the phosphoenolpyruvate carboxylase encoded by  pepC catalyzing the conversion of phosphoenolpyruvate to oxaloacetate as one of the anaplerotic reactions was also overexpressed to augment the utilization of carbohydrates and to ultimately increase the metabolic flux towards 2-oxoglutarate, which is the substrate for glutamate and subsequently arginine biosynthesis.	transcription
52405	8	334961	5	NULL	NULL	0	NULL	2-oxoglutarate	NULL		is a substrate for	NULL				glutamate	NULL				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_2_1410_s_162	16461694	Since CGP biosynthesis in cells of  Acinetobacter sp. strain ADP1 using sugars or other carbohydrates as substrates gave only low amounts of CGP and since it was recently reported that  Acinetobacter sp. strain ADP1 is lacking a gene encoding pyruvate kinase, which is involved in the conversion of carbohydrates to pyruvate ( ), the phosphoenolpyruvate carboxylase encoded by  pepC catalyzing the conversion of phosphoenolpyruvate to oxaloacetate as one of the anaplerotic reactions was also overexpressed to augment the utilization of carbohydrates and to ultimately increase the metabolic flux towards 2-oxoglutarate, which is the substrate for glutamate and subsequently arginine biosynthesis.	transcription
52406	9	334961	5	NULL	NULL	0	NULL	2-oxoglutarate	NULL		is required for	NULL				arginine	NULL	biosynthesis of			NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_2_1410_s_162	16461694	Since CGP biosynthesis in cells of  Acinetobacter sp. strain ADP1 using sugars or other carbohydrates as substrates gave only low amounts of CGP and since it was recently reported that  Acinetobacter sp. strain ADP1 is lacking a gene encoding pyruvate kinase, which is involved in the conversion of carbohydrates to pyruvate ( ), the phosphoenolpyruvate carboxylase encoded by  pepC catalyzing the conversion of phosphoenolpyruvate to oxaloacetate as one of the anaplerotic reactions was also overexpressed to augment the utilization of carbohydrates and to ultimately increase the metabolic flux towards 2-oxoglutarate, which is the substrate for glutamate and subsequently arginine biosynthesis.	transcription
55620	1	334961	6	NULL	NULL	0	NULL	Acinetobacter sp. strain ADP1			lacks					pyruvate kinase gene					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_2_1410_s_162	16461694	Since CGP biosynthesis in cells of  Acinetobacter sp. strain ADP1 using sugars or other carbohydrates as substrates gave only low amounts of CGP and since it was recently reported that  Acinetobacter sp. strain ADP1 is lacking a gene encoding pyruvate kinase, which is involved in the conversion of carbohydrates to pyruvate ( ), the phosphoenolpyruvate carboxylase encoded by  pepC catalyzing the conversion of phosphoenolpyruvate to oxaloacetate as one of the anaplerotic reactions was also overexpressed to augment the utilization of carbohydrates and to ultimately increase the metabolic flux towards 2-oxoglutarate, which is the substrate for glutamate and subsequently arginine biosynthesis.	transcription
55621	2	334961	6	NULL	NULL	0	NULL	carbohydrate			is converted to					pyruvate					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_2_1410_s_162	16461694	Since CGP biosynthesis in cells of  Acinetobacter sp. strain ADP1 using sugars or other carbohydrates as substrates gave only low amounts of CGP and since it was recently reported that  Acinetobacter sp. strain ADP1 is lacking a gene encoding pyruvate kinase, which is involved in the conversion of carbohydrates to pyruvate ( ), the phosphoenolpyruvate carboxylase encoded by  pepC catalyzing the conversion of phosphoenolpyruvate to oxaloacetate as one of the anaplerotic reactions was also overexpressed to augment the utilization of carbohydrates and to ultimately increase the metabolic flux towards 2-oxoglutarate, which is the substrate for glutamate and subsequently arginine biosynthesis.	transcription
55622	3	334961	6	NULL	NULL	0	NULL	pyruvate kinase			is involved in					statement 2					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_2_1410_s_162	16461694	Since CGP biosynthesis in cells of  Acinetobacter sp. strain ADP1 using sugars or other carbohydrates as substrates gave only low amounts of CGP and since it was recently reported that  Acinetobacter sp. strain ADP1 is lacking a gene encoding pyruvate kinase, which is involved in the conversion of carbohydrates to pyruvate ( ), the phosphoenolpyruvate carboxylase encoded by  pepC catalyzing the conversion of phosphoenolpyruvate to oxaloacetate as one of the anaplerotic reactions was also overexpressed to augment the utilization of carbohydrates and to ultimately increase the metabolic flux towards 2-oxoglutarate, which is the substrate for glutamate and subsequently arginine biosynthesis.	transcription
55623	4	334961	6	NULL	NULL	0	NULL	pepC			encodes for					phosphoenolpyruvate carboxylase					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_2_1410_s_162	16461694	Since CGP biosynthesis in cells of  Acinetobacter sp. strain ADP1 using sugars or other carbohydrates as substrates gave only low amounts of CGP and since it was recently reported that  Acinetobacter sp. strain ADP1 is lacking a gene encoding pyruvate kinase, which is involved in the conversion of carbohydrates to pyruvate ( ), the phosphoenolpyruvate carboxylase encoded by  pepC catalyzing the conversion of phosphoenolpyruvate to oxaloacetate as one of the anaplerotic reactions was also overexpressed to augment the utilization of carbohydrates and to ultimately increase the metabolic flux towards 2-oxoglutarate, which is the substrate for glutamate and subsequently arginine biosynthesis.	transcription
55624	5	334961	6	NULL	NULL	0	NULL	Phosphoenolpyruvate			is converted to					oxaloacetate					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_2_1410_s_162	16461694	Since CGP biosynthesis in cells of  Acinetobacter sp. strain ADP1 using sugars or other carbohydrates as substrates gave only low amounts of CGP and since it was recently reported that  Acinetobacter sp. strain ADP1 is lacking a gene encoding pyruvate kinase, which is involved in the conversion of carbohydrates to pyruvate ( ), the phosphoenolpyruvate carboxylase encoded by  pepC catalyzing the conversion of phosphoenolpyruvate to oxaloacetate as one of the anaplerotic reactions was also overexpressed to augment the utilization of carbohydrates and to ultimately increase the metabolic flux towards 2-oxoglutarate, which is the substrate for glutamate and subsequently arginine biosynthesis.	transcription
55625	6	334961	6	NULL	NULL	0	NULL	pepC			catalyzes					statement 5					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_2_1410_s_162	16461694	Since CGP biosynthesis in cells of  Acinetobacter sp. strain ADP1 using sugars or other carbohydrates as substrates gave only low amounts of CGP and since it was recently reported that  Acinetobacter sp. strain ADP1 is lacking a gene encoding pyruvate kinase, which is involved in the conversion of carbohydrates to pyruvate ( ), the phosphoenolpyruvate carboxylase encoded by  pepC catalyzing the conversion of phosphoenolpyruvate to oxaloacetate as one of the anaplerotic reactions was also overexpressed to augment the utilization of carbohydrates and to ultimately increase the metabolic flux towards 2-oxoglutarate, which is the substrate for glutamate and subsequently arginine biosynthesis.	transcription
52407	1	334962	5	NULL	NULL	0	NULL	alanine	NULL		connected to	NULL	directly			pyruvate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_46_47881_s_180	15361523	Indeed, alanine is directly connected with pyruvate through aminotransferase activity, whereas the metabolic pathways leading to the other amino acids involve multisteps (the carbon in the pyruvate C3 position gives the C2 of acetyl-CoA, which becomes the C4 of 2-oxoglutarate and, further, the C3 or C2 of oxaloacetate in the first tricarboxylic acid cycle turn; from these intermediates, the carbon may be recovered either at glutamate C4, glutamine C4, GABA C2, or aspartate C2 or C3).	transcription
52408	2	334962	5	NULL	NULL	0	NULL	statement 1	NULL		occurs through	NULL				aminotransferase	NULL	activity of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_46_47881_s_180	15361523	Indeed, alanine is directly connected with pyruvate through aminotransferase activity, whereas the metabolic pathways leading to the other amino acids involve multisteps (the carbon in the pyruvate C3 position gives the C2 of acetyl-CoA, which becomes the C4 of 2-oxoglutarate and, further, the C3 or C2 of oxaloacetate in the first tricarboxylic acid cycle turn; from these intermediates, the carbon may be recovered either at glutamate C4, glutamine C4, GABA C2, or aspartate C2 or C3).	transcription
55325	1	334962	6	NULL	NULL	0	NULL	alanine			is connected to					pyruvate					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_46_47881_s_180	15361523	Indeed, alanine is directly connected with pyruvate through aminotransferase activity, whereas the metabolic pathways leading to the other amino acids involve multisteps (the carbon in the pyruvate C3 position gives the C2 of acetyl-CoA, which becomes the C4 of 2-oxoglutarate and, further, the C3 or C2 of oxaloacetate in the first tricarboxylic acid cycle turn; from these intermediates, the carbon may be recovered either at glutamate C4, glutamine C4, GABA C2, or aspartate C2 or C3).	transcription
55326	2	334962	6	NULL	NULL	0	NULL	statement 1			occurs through					aminotransferase activity					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_46_47881_s_180	15361523	Indeed, alanine is directly connected with pyruvate through aminotransferase activity, whereas the metabolic pathways leading to the other amino acids involve multisteps (the carbon in the pyruvate C3 position gives the C2 of acetyl-CoA, which becomes the C4 of 2-oxoglutarate and, further, the C3 or C2 of oxaloacetate in the first tricarboxylic acid cycle turn; from these intermediates, the carbon may be recovered either at glutamate C4, glutamine C4, GABA C2, or aspartate C2 or C3).	transcription
52420	1	334963	5	NULL	NULL	0	NULL	accA3	NULL		is a subunit of	NULL				acetyl CoA carboxylase	NULL				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_2_467_s_120	15626759	The two smaller species were identified as the biotin-containing subunit of acetyl CoA carboxylase (encoded by  accA3), which catalyzes the conversion of acetyl CoA to malonyl CoA, the first committed step in fatty acid biosynthesis, and pyruvate carboxylase (encoded by  pca), which catalyzes the conversion of pyruvate to oxaloacetate and serves an essential anaplerotic role during periods of metabolic shunting.	transcription
52421	2	334963	5	NULL	NULL	0	NULL	accA3	NULL		contains	NULL				biotin	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_2_467_s_120	15626759	The two smaller species were identified as the biotin-containing subunit of acetyl CoA carboxylase (encoded by  accA3), which catalyzes the conversion of acetyl CoA to malonyl CoA, the first committed step in fatty acid biosynthesis, and pyruvate carboxylase (encoded by  pca), which catalyzes the conversion of pyruvate to oxaloacetate and serves an essential anaplerotic role during periods of metabolic shunting.	transcription
52422	3	334963	5	NULL	NULL	0	NULL	acetyl CoA	NULL		is converted to	NULL				malonyl CoA	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_2_467_s_120	15626759	The two smaller species were identified as the biotin-containing subunit of acetyl CoA carboxylase (encoded by  accA3), which catalyzes the conversion of acetyl CoA to malonyl CoA, the first committed step in fatty acid biosynthesis, and pyruvate carboxylase (encoded by  pca), which catalyzes the conversion of pyruvate to oxaloacetate and serves an essential anaplerotic role during periods of metabolic shunting.	transcription
52423	4	334963	5	NULL	NULL	0	NULL	acetyl CoA carboxylase	NULL		catalyzes	NULL		accA3		statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_2_467_s_120	15626759	The two smaller species were identified as the biotin-containing subunit of acetyl CoA carboxylase (encoded by  accA3), which catalyzes the conversion of acetyl CoA to malonyl CoA, the first committed step in fatty acid biosynthesis, and pyruvate carboxylase (encoded by  pca), which catalyzes the conversion of pyruvate to oxaloacetate and serves an essential anaplerotic role during periods of metabolic shunting.	transcription
52424	5	334963	5	NULL	NULL	0	NULL	pyruvate carboxylase	NULL		is encoded by	NULL				pca	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_2_467_s_120	15626759	The two smaller species were identified as the biotin-containing subunit of acetyl CoA carboxylase (encoded by  accA3), which catalyzes the conversion of acetyl CoA to malonyl CoA, the first committed step in fatty acid biosynthesis, and pyruvate carboxylase (encoded by  pca), which catalyzes the conversion of pyruvate to oxaloacetate and serves an essential anaplerotic role during periods of metabolic shunting.	transcription
52425	6	334963	5	NULL	NULL	0	NULL	pyruvate	NULL		is converted to	NULL				oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_2_467_s_120	15626759	The two smaller species were identified as the biotin-containing subunit of acetyl CoA carboxylase (encoded by  accA3), which catalyzes the conversion of acetyl CoA to malonyl CoA, the first committed step in fatty acid biosynthesis, and pyruvate carboxylase (encoded by  pca), which catalyzes the conversion of pyruvate to oxaloacetate and serves an essential anaplerotic role during periods of metabolic shunting.	transcription
52426	7	334963	5	NULL	NULL	0	NULL	pca	NULL		catalyzes	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw70_pnas_102_2_467_s_120	15626759	The two smaller species were identified as the biotin-containing subunit of acetyl CoA carboxylase (encoded by  accA3), which catalyzes the conversion of acetyl CoA to malonyl CoA, the first committed step in fatty acid biosynthesis, and pyruvate carboxylase (encoded by  pca), which catalyzes the conversion of pyruvate to oxaloacetate and serves an essential anaplerotic role during periods of metabolic shunting.	transcription
52427	8	334963	5	NULL	NULL	0	NULL	pca	NULL		serves as	NULL				anaplerotic	NULL	essential			NULL		0	NULL	NULL	NULL	gw70_pnas_102_2_467_s_120	15626759	The two smaller species were identified as the biotin-containing subunit of acetyl CoA carboxylase (encoded by  accA3), which catalyzes the conversion of acetyl CoA to malonyl CoA, the first committed step in fatty acid biosynthesis, and pyruvate carboxylase (encoded by  pca), which catalyzes the conversion of pyruvate to oxaloacetate and serves an essential anaplerotic role during periods of metabolic shunting.	transcription
52428	9	334963	5	NULL	NULL	0	NULL	statement 8	NULL		occurs during	NULL				metabolic shunting	NULL	periods of 			NULL		0	NULL	NULL	NULL	gw70_pnas_102_2_467_s_120	15626759	The two smaller species were identified as the biotin-containing subunit of acetyl CoA carboxylase (encoded by  accA3), which catalyzes the conversion of acetyl CoA to malonyl CoA, the first committed step in fatty acid biosynthesis, and pyruvate carboxylase (encoded by  pca), which catalyzes the conversion of pyruvate to oxaloacetate and serves an essential anaplerotic role during periods of metabolic shunting.	transcription
52429	10	334963	5	NULL	NULL	0	NULL	statement 4	NULL		leads to	NULL				fatty acids	NULL	biosynthesis of			NULL		0	NULL	NULL	NULL	gw70_pnas_102_2_467_s_120	15626759	The two smaller species were identified as the biotin-containing subunit of acetyl CoA carboxylase (encoded by  accA3), which catalyzes the conversion of acetyl CoA to malonyl CoA, the first committed step in fatty acid biosynthesis, and pyruvate carboxylase (encoded by  pca), which catalyzes the conversion of pyruvate to oxaloacetate and serves an essential anaplerotic role during periods of metabolic shunting.	transcription
55329	1	334963	6	NULL	NULL	0	NULL	acetyl CoA			is converted to					malonyl CoA					NULL		0	NULL	NULL	NULL	gw70_pnas_102_2_467_s_120	15626759	The two smaller species were identified as the biotin-containing subunit of acetyl CoA carboxylase (encoded by  accA3), which catalyzes the conversion of acetyl CoA to malonyl CoA, the first committed step in fatty acid biosynthesis, and pyruvate carboxylase (encoded by  pca), which catalyzes the conversion of pyruvate to oxaloacetate and serves an essential anaplerotic role during periods of metabolic shunting.	transcription
55331	2	334963	6	NULL	NULL	0	NULL	statement 1			occurs in					fatty acid		biosynthesis of 			NULL		0	NULL	NULL	NULL	gw70_pnas_102_2_467_s_120	15626759	The two smaller species were identified as the biotin-containing subunit of acetyl CoA carboxylase (encoded by  accA3), which catalyzes the conversion of acetyl CoA to malonyl CoA, the first committed step in fatty acid biosynthesis, and pyruvate carboxylase (encoded by  pca), which catalyzes the conversion of pyruvate to oxaloacetate and serves an essential anaplerotic role during periods of metabolic shunting.	transcription
55347	3	334963	6	NULL	NULL	0	NULL	accA3			is					acetyl CoA carboxylase					NULL		0	NULL	NULL	NULL	gw70_pnas_102_2_467_s_120	15626759	The two smaller species were identified as the biotin-containing subunit of acetyl CoA carboxylase (encoded by  accA3), which catalyzes the conversion of acetyl CoA to malonyl CoA, the first committed step in fatty acid biosynthesis, and pyruvate carboxylase (encoded by  pca), which catalyzes the conversion of pyruvate to oxaloacetate and serves an essential anaplerotic role during periods of metabolic shunting.	transcription
55356	4	334963	6	NULL	NULL	0	NULL	pca			is					pyruvate carboxylase					NULL		0	NULL	NULL	NULL	gw70_pnas_102_2_467_s_120	15626759	The two smaller species were identified as the biotin-containing subunit of acetyl CoA carboxylase (encoded by  accA3), which catalyzes the conversion of acetyl CoA to malonyl CoA, the first committed step in fatty acid biosynthesis, and pyruvate carboxylase (encoded by  pca), which catalyzes the conversion of pyruvate to oxaloacetate and serves an essential anaplerotic role during periods of metabolic shunting.	transcription
55357	5	334963	6	NULL	NULL	0	NULL	pyruvate			is converted to					oxaloacetate					NULL		0	NULL	NULL	NULL	gw70_pnas_102_2_467_s_120	15626759	The two smaller species were identified as the biotin-containing subunit of acetyl CoA carboxylase (encoded by  accA3), which catalyzes the conversion of acetyl CoA to malonyl CoA, the first committed step in fatty acid biosynthesis, and pyruvate carboxylase (encoded by  pca), which catalyzes the conversion of pyruvate to oxaloacetate and serves an essential anaplerotic role during periods of metabolic shunting.	transcription
55359	6	334963	6	NULL	NULL	0	NULL	pca			catalyzes					statement 5					NULL		0	NULL	NULL	NULL	gw70_pnas_102_2_467_s_120	15626759	The two smaller species were identified as the biotin-containing subunit of acetyl CoA carboxylase (encoded by  accA3), which catalyzes the conversion of acetyl CoA to malonyl CoA, the first committed step in fatty acid biosynthesis, and pyruvate carboxylase (encoded by  pca), which catalyzes the conversion of pyruvate to oxaloacetate and serves an essential anaplerotic role during periods of metabolic shunting.	transcription
52409	1	334964	5	NULL	NULL	0	NULL	glycolate	NULL	provision of energy from	occur via	NULL	may			dicarboxylic acid cycle	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_9993_s_54	12556462	Jack and I were able to show that the provision of energy from glycolate could occur  via a dicarboxylic acid cycle, in which an isoform of malate synthetase catalyzed the condensation of glyoxylate and acetyl-coenzyme A as the first step in a sequence of reactions that led from malate via oxaloacetate and pyruvate to the loss of two carbons as CO2 and to the reformation of the acetyl-coenzyme A acceptor ( ).	transcription
52410	2	334964	5	NULL	NULL	0	NULL	isoform of malate synthetase	NULL		catalyzes	NULL				glyoxylate	NULL	condensation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_9993_s_54	12556462	Jack and I were able to show that the provision of energy from glycolate could occur  via a dicarboxylic acid cycle, in which an isoform of malate synthetase catalyzed the condensation of glyoxylate and acetyl-coenzyme A as the first step in a sequence of reactions that led from malate via oxaloacetate and pyruvate to the loss of two carbons as CO2 and to the reformation of the acetyl-coenzyme A acceptor ( ).	transcription
52411	3	334964	5	NULL	NULL	0	NULL	isoform of malate synthetase	NULL		catalyzes	NULL				acetyl-coenzyme A 	NULL	condensation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_9993_s_54	12556462	Jack and I were able to show that the provision of energy from glycolate could occur  via a dicarboxylic acid cycle, in which an isoform of malate synthetase catalyzed the condensation of glyoxylate and acetyl-coenzyme A as the first step in a sequence of reactions that led from malate via oxaloacetate and pyruvate to the loss of two carbons as CO2 and to the reformation of the acetyl-coenzyme A acceptor ( ).	transcription
52412	4	334964	5	NULL	NULL	0	NULL	statement 2	NULL		occurs along with	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_9993_s_54	12556462	Jack and I were able to show that the provision of energy from glycolate could occur  via a dicarboxylic acid cycle, in which an isoform of malate synthetase catalyzed the condensation of glyoxylate and acetyl-coenzyme A as the first step in a sequence of reactions that led from malate via oxaloacetate and pyruvate to the loss of two carbons as CO2 and to the reformation of the acetyl-coenzyme A acceptor ( ).	transcription
52413	5	334964	5	NULL	NULL	0	NULL	statement 4	NULL		led from	NULL				malate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_9993_s_54	12556462	Jack and I were able to show that the provision of energy from glycolate could occur  via a dicarboxylic acid cycle, in which an isoform of malate synthetase catalyzed the condensation of glyoxylate and acetyl-coenzyme A as the first step in a sequence of reactions that led from malate via oxaloacetate and pyruvate to the loss of two carbons as CO2 and to the reformation of the acetyl-coenzyme A acceptor ( ).	transcription
52414	6	334964	5	NULL	NULL	0	NULL	carbon	NULL		is lost as	NULL				CO2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_9993_s_54	12556462	Jack and I were able to show that the provision of energy from glycolate could occur  via a dicarboxylic acid cycle, in which an isoform of malate synthetase catalyzed the condensation of glyoxylate and acetyl-coenzyme A as the first step in a sequence of reactions that led from malate via oxaloacetate and pyruvate to the loss of two carbons as CO2 and to the reformation of the acetyl-coenzyme A acceptor ( ).	transcription
52415	7	334964	5	NULL	NULL	0	NULL	statement 4	NULL		led to	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_9993_s_54	12556462	Jack and I were able to show that the provision of energy from glycolate could occur  via a dicarboxylic acid cycle, in which an isoform of malate synthetase catalyzed the condensation of glyoxylate and acetyl-coenzyme A as the first step in a sequence of reactions that led from malate via oxaloacetate and pyruvate to the loss of two carbons as CO2 and to the reformation of the acetyl-coenzyme A acceptor ( ).	transcription
52416	8	334964	5	NULL	NULL	0	NULL	statement 7	NULL		via	NULL				oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_9993_s_54	12556462	Jack and I were able to show that the provision of energy from glycolate could occur  via a dicarboxylic acid cycle, in which an isoform of malate synthetase catalyzed the condensation of glyoxylate and acetyl-coenzyme A as the first step in a sequence of reactions that led from malate via oxaloacetate and pyruvate to the loss of two carbons as CO2 and to the reformation of the acetyl-coenzyme A acceptor ( ).	transcription
52417	9	334964	5	NULL	NULL	0	NULL	statement 7	NULL		via	NULL				pyruvate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_9993_s_54	12556462	Jack and I were able to show that the provision of energy from glycolate could occur  via a dicarboxylic acid cycle, in which an isoform of malate synthetase catalyzed the condensation of glyoxylate and acetyl-coenzyme A as the first step in a sequence of reactions that led from malate via oxaloacetate and pyruvate to the loss of two carbons as CO2 and to the reformation of the acetyl-coenzyme A acceptor ( ).	transcription
52418	10	334964	5	NULL	NULL	0	NULL	statement 7	NULL		led to	NULL				acetyl-coenzyme A acceptor	NULL	reformation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_9993_s_54	12556462	Jack and I were able to show that the provision of energy from glycolate could occur  via a dicarboxylic acid cycle, in which an isoform of malate synthetase catalyzed the condensation of glyoxylate and acetyl-coenzyme A as the first step in a sequence of reactions that led from malate via oxaloacetate and pyruvate to the loss of two carbons as CO2 and to the reformation of the acetyl-coenzyme A acceptor ( ).	transcription
52430	1	334966	5	NULL	NULL	0	NULL	liver tumor	NULL		is induced by	NULL				DEN	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
52431	2	334966	5	NULL	NULL	0	NULL	Bauhinia variegata	NULL	extract of	suppress	NULL	effectively			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
52432	3	334966	5	NULL	NULL	0	NULL	DEN	NULL		induce	NULL				SGPT	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
52433	4	334966	5	NULL	NULL	0	NULL	SGPT	NULL		is	NULL				serum glutamate pyruvate transaminase	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
52434	5	334966	5	NULL	NULL	0	NULL	SGOT	NULL		is	NULL				serum glutamate oxaloacetate transaminase	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
52435	6	334966	5	NULL	NULL	0	NULL	DEN	NULL		induce	NULL				SGOT	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
52436	7	334966	5	NULL	NULL	0	NULL	DEN	NULL		induce	NULL				ALP	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
52437	8	334966	5	NULL	NULL	0	NULL	ALP	NULL		is	NULL				alkaline phosphatase	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
52438	9	334966	5	NULL	NULL	0	NULL	DEN	NULL		induce	NULL				bilirubin	NULL	total			NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
52439	10	334966	5	NULL	NULL	0	NULL	DEN	NULL		induce	NULL				GGTP	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
52440	11	334966	5	NULL	NULL	0	NULL	GGTP	NULL		is	NULL				gamma glutamate transpeptidase	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
52441	12	334966	5	NULL	NULL	0	NULL	DEN	NULL		induce	NULL				LPO	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
52442	13	334966	5	NULL	NULL	0	NULL	LPO	NULL		is	NULL				lipid peroxidase	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
52443	14	334966	5	NULL	NULL	0	NULL	DEN	NULL		induce	NULL				GPx	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
52444	15	334966	5	NULL	NULL	0	NULL	GPx	NULL		is	NULL				glutathione peroxidase	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
52445	16	334966	5	NULL	NULL	0	NULL	DEN	NULL		induce	NULL				GST	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
52446	17	334966	5	NULL	NULL	0	NULL	GST	NULL		is	NULL				glutathione S-transferase	NULL				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
55373	1	334966	6	NULL	NULL	0	NULL	DEN			induces					liver tumor					NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
55374	2	334966	6	NULL	NULL	0	NULL	Bauhinia variegata extracts			suppress					statement 1					NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
55375	3	334966	6	NULL	NULL	0	NULL	DEN			induces					SGPT		elevated levels of 			NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
55377	4	334966	6	NULL	NULL	0	NULL	Bauhinia variegata extracts		administration of	decreases					statement 3					NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
55378	5	334966	6	NULL	NULL	0	NULL	SGPT			is					serum glutamate pyruvate transaminase					NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
55379	6	334966	6	NULL	NULL	0	NULL	SGOT			is					serum glutamate oxaloacetate transaminase					NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
55380	7	334966	6	NULL	NULL	0	NULL	DEN			induces					SGOT		elevated levels of			NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
55381	8	334966	6	NULL	NULL	0	NULL	Bauhinia variegata extracts		administration of	decreases					statement 7					NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
55386	9	334966	6	NULL	NULL	0	NULL	DEN			induces					ALP					NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
55388	10	334966	6	NULL	NULL	0	NULL	Bauhinia variegata extracts		administration of	decreases					statement 9					NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
55389	11	334966	6	NULL	NULL	0	NULL	ALP			is					alkaline phosphatase					NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
55396	12	334966	6	NULL	NULL	0	NULL	DEN			induces					total bilirubin		elevated levels of			NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
55399	13	334966	6	NULL	NULL	0	NULL	Bauhinia variegata extracts		administration of	decreases					statement 12					NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
55400	14	334966	6	NULL	NULL	0	NULL	DEN			induces					GGTP		elevated levels of			NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
55401	15	334966	6	NULL	NULL	0	NULL	GGTP			is					gamma glutamate transpeptidase					NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
55402	16	334966	6	NULL	NULL	0	NULL	Bauhinia variegata extracts		administration of	decreases					statement 14					NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
55403	17	334966	6	NULL	NULL	0	NULL	LPO			is					lipid peroxidase					NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
55409	18	334966	6	NULL	NULL	0	NULL	DEN			induces					LPO		elevated levels of			NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
55410	19	334966	6	NULL	NULL	0	NULL	Bauhinia variegata extracts		administration of	decreases					statement 18					NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
55411	20	334966	6	NULL	NULL	0	NULL	GPx			is					glutathione peroxidase					NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
55412	21	334966	6	NULL	NULL	0	NULL	DEN			induces					GPx		elevated levels of			NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
55413	22	334966	6	NULL	NULL	0	NULL	Bauhinia variegata extracts		administration of	decreases					statement 18					NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-ethnopharmacol_104_3_16257158_s_3	16257158	Oral administration of ethanol extract of Bauhinia variegata (250mg/kg)  effectively suppressed liver tumor induced by DEN as revealed by decrease  in DEN induced elevated levels of serum glutamate pyruvate transaminase  (SGPT), serum glutamate oxaloacetate transaminase (SGOT), alkaline phosphatase  (ALP), total bilirubin, gamma glutamate transpeptidase (GGTP), lipid peroxidase  (LPO), glutathione peroxidase (GPx) and glutathione S-transferase (GST).	transcription
52447	1	334968	5	NULL	NULL	0	NULL	ATP	NULL		bind	NULL				PII	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_8_2582_s_23	12670983	Conversely, the binding of ATP to PII inhibits phospho-PII dephosphorylation; this inhibition is greatly enhanced by 2-oxoglutarate and to a lesser extent by oxaloacetate ( ).	transcription
52448	2	334968	5	NULL	NULL	0	NULL	statement 1	NULL		inhibit	NULL				phospho-PII	NULL	dephosphorylation of			NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_8_2582_s_23	12670983	Conversely, the binding of ATP to PII inhibits phospho-PII dephosphorylation; this inhibition is greatly enhanced by 2-oxoglutarate and to a lesser extent by oxaloacetate ( ).	transcription
52449	3	334968	5	NULL	NULL	0	NULL	2-oxoglutarate	NULL		enhance	NULL	greatly			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_8_2582_s_23	12670983	Conversely, the binding of ATP to PII inhibits phospho-PII dephosphorylation; this inhibition is greatly enhanced by 2-oxoglutarate and to a lesser extent by oxaloacetate ( ).	transcription
52450	4	334968	5	NULL	NULL	0	NULL	oxaloacetate	NULL		enhance	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_8_2582_s_23	12670983	Conversely, the binding of ATP to PII inhibits phospho-PII dephosphorylation; this inhibition is greatly enhanced by 2-oxoglutarate and to a lesser extent by oxaloacetate ( ).	transcription
55415	1	334968	6	NULL	NULL	0	NULL	ATP			bind					PII					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_8_2582_s_23	12670983	Conversely, the binding of ATP to PII inhibits phospho-PII dephosphorylation; this inhibition is greatly enhanced by 2-oxoglutarate and to a lesser extent by oxaloacetate ( ).	transcription
55417	2	334968	6	NULL	NULL	0	NULL	statement 1			inhibits					phospho-PII		dephosphorylation of 			NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_8_2582_s_23	12670983	Conversely, the binding of ATP to PII inhibits phospho-PII dephosphorylation; this inhibition is greatly enhanced by 2-oxoglutarate and to a lesser extent by oxaloacetate ( ).	transcription
55420	3	334968	6	NULL	NULL	0	NULL	statement 2			is enhanced by					2-oxoglutarate					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_8_2582_s_23	12670983	Conversely, the binding of ATP to PII inhibits phospho-PII dephosphorylation; this inhibition is greatly enhanced by 2-oxoglutarate and to a lesser extent by oxaloacetate ( ).	transcription
55471	4	334968	6	NULL	NULL	0	NULL	statement 2			is enhanced by					oxaloacetate					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_185_8_2582_s_23	12670983	Conversely, the binding of ATP to PII inhibits phospho-PII dephosphorylation; this inhibition is greatly enhanced by 2-oxoglutarate and to a lesser extent by oxaloacetate ( ).	transcription
52451	1	334969	5	NULL	NULL	0	NULL	NtcA	NULL		bind	NULL				glnA	NULL	Synechococcus		promoter	NULL		0	NULL	NULL	NULL	gw60_febslett_512_1_71_s_69	11852054	Effect of different concentrations of 2-oxoglutarate, 3-oxoglutarate, glutamate or oxaloacetate on the binding of NtcA to the  Synechococcus glnA promoter.	transcription
55472	1	334969	6	NULL	NULL	0	NULL	NtcA			bind					glnA		Synechococcus		promoter	NULL		0	NULL	NULL	NULL	gw60_febslett_512_1_71_s_69	11852054	Effect of different concentrations of 2-oxoglutarate, 3-oxoglutarate, glutamate or oxaloacetate on the binding of NtcA to the  Synechococcus glnA promoter.	transcription
52452	1	334970	5	NULL	NULL	0	NULL	succinyl-CoA	NULL		is carboxylated to	NULL				2-oxoglutarate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_9_3020_s_23	15838028	2-Oxoglutarate:ferredoxin oxidoreductase catalyzes the carboxylation of succinyl-CoA to 2-oxoglutarate, ATP citrate lyase the ATP-dependent cleavage of citrate to acetyl-CoA and oxaloacetate, and fumarate reductase the reduction of fumarate forming succinate.	transcription
52453	2	334970	5	NULL	NULL	0	NULL	2-Oxoglutarate:ferredoxin oxidoreductase	NULL		catalyzes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_9_3020_s_23	15838028	2-Oxoglutarate:ferredoxin oxidoreductase catalyzes the carboxylation of succinyl-CoA to 2-oxoglutarate, ATP citrate lyase the ATP-dependent cleavage of citrate to acetyl-CoA and oxaloacetate, and fumarate reductase the reduction of fumarate forming succinate.	transcription
52454	3	334970	5	NULL	NULL	0	NULL	citrate	NULL		is cleaved into	NULL				acetyl-CoA	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_9_3020_s_23	15838028	2-Oxoglutarate:ferredoxin oxidoreductase catalyzes the carboxylation of succinyl-CoA to 2-oxoglutarate, ATP citrate lyase the ATP-dependent cleavage of citrate to acetyl-CoA and oxaloacetate, and fumarate reductase the reduction of fumarate forming succinate.	transcription
52455	4	334970	5	NULL	NULL	0	NULL	citrate	NULL		is cleaved into	NULL				oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_9_3020_s_23	15838028	2-Oxoglutarate:ferredoxin oxidoreductase catalyzes the carboxylation of succinyl-CoA to 2-oxoglutarate, ATP citrate lyase the ATP-dependent cleavage of citrate to acetyl-CoA and oxaloacetate, and fumarate reductase the reduction of fumarate forming succinate.	transcription
52456	5	334970	5	NULL	NULL	0	NULL	statement 3	NULL		occurs along with	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_9_3020_s_23	15838028	2-Oxoglutarate:ferredoxin oxidoreductase catalyzes the carboxylation of succinyl-CoA to 2-oxoglutarate, ATP citrate lyase the ATP-dependent cleavage of citrate to acetyl-CoA and oxaloacetate, and fumarate reductase the reduction of fumarate forming succinate.	transcription
52457	6	334970	5	NULL	NULL	0	NULL	statement 5	NULL		is dependent on	NULL				ATP	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_9_3020_s_23	15838028	2-Oxoglutarate:ferredoxin oxidoreductase catalyzes the carboxylation of succinyl-CoA to 2-oxoglutarate, ATP citrate lyase the ATP-dependent cleavage of citrate to acetyl-CoA and oxaloacetate, and fumarate reductase the reduction of fumarate forming succinate.	transcription
52458	7	334970	5	NULL	NULL	0	NULL	ATP citrate lyase	NULL		catalyzes	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_9_3020_s_23	15838028	2-Oxoglutarate:ferredoxin oxidoreductase catalyzes the carboxylation of succinyl-CoA to 2-oxoglutarate, ATP citrate lyase the ATP-dependent cleavage of citrate to acetyl-CoA and oxaloacetate, and fumarate reductase the reduction of fumarate forming succinate.	transcription
52459	8	334970	5	NULL	NULL	0	NULL	fumarate	NULL	reduction of	leads to	NULL				succinate	NULL	formation of			NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_9_3020_s_23	15838028	2-Oxoglutarate:ferredoxin oxidoreductase catalyzes the carboxylation of succinyl-CoA to 2-oxoglutarate, ATP citrate lyase the ATP-dependent cleavage of citrate to acetyl-CoA and oxaloacetate, and fumarate reductase the reduction of fumarate forming succinate.	transcription
52460	9	334970	5	NULL	NULL	0	NULL	fumarate reductase	NULL		catalyzes	NULL				statement 8	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_9_3020_s_23	15838028	2-Oxoglutarate:ferredoxin oxidoreductase catalyzes the carboxylation of succinyl-CoA to 2-oxoglutarate, ATP citrate lyase the ATP-dependent cleavage of citrate to acetyl-CoA and oxaloacetate, and fumarate reductase the reduction of fumarate forming succinate.	transcription
55473	1	334970	6	NULL	NULL	0	NULL	succinyl-CoA			is carboxylated to					2-oxoglutarate					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_9_3020_s_23	15838028	2-Oxoglutarate:ferredoxin oxidoreductase catalyzes the carboxylation of succinyl-CoA to 2-oxoglutarate, ATP citrate lyase the ATP-dependent cleavage of citrate to acetyl-CoA and oxaloacetate, and fumarate reductase the reduction of fumarate forming succinate.	transcription
55474	2	334970	6	NULL	NULL	0	NULL	2-Oxoglutarate:ferredoxin oxidoreductase			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_9_3020_s_23	15838028	2-Oxoglutarate:ferredoxin oxidoreductase catalyzes the carboxylation of succinyl-CoA to 2-oxoglutarate, ATP citrate lyase the ATP-dependent cleavage of citrate to acetyl-CoA and oxaloacetate, and fumarate reductase the reduction of fumarate forming succinate.	transcription
55475	3	334970	6	NULL	NULL	0	NULL	citrate			is converted to					acetyl-CoA					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_9_3020_s_23	15838028	2-Oxoglutarate:ferredoxin oxidoreductase catalyzes the carboxylation of succinyl-CoA to 2-oxoglutarate, ATP citrate lyase the ATP-dependent cleavage of citrate to acetyl-CoA and oxaloacetate, and fumarate reductase the reduction of fumarate forming succinate.	transcription
55476	4	334970	6	NULL	NULL	0	NULL	citrate			is converted to					oxaloacetate					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_9_3020_s_23	15838028	2-Oxoglutarate:ferredoxin oxidoreductase catalyzes the carboxylation of succinyl-CoA to 2-oxoglutarate, ATP citrate lyase the ATP-dependent cleavage of citrate to acetyl-CoA and oxaloacetate, and fumarate reductase the reduction of fumarate forming succinate.	transcription
55477	5	334970	6	NULL	NULL	0	NULL	statement 3			is dependent on					ATP					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_9_3020_s_23	15838028	2-Oxoglutarate:ferredoxin oxidoreductase catalyzes the carboxylation of succinyl-CoA to 2-oxoglutarate, ATP citrate lyase the ATP-dependent cleavage of citrate to acetyl-CoA and oxaloacetate, and fumarate reductase the reduction of fumarate forming succinate.	transcription
55478	6	334970	6	NULL	NULL	0	NULL	statement 4			is dependent on					ATP					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_9_3020_s_23	15838028	2-Oxoglutarate:ferredoxin oxidoreductase catalyzes the carboxylation of succinyl-CoA to 2-oxoglutarate, ATP citrate lyase the ATP-dependent cleavage of citrate to acetyl-CoA and oxaloacetate, and fumarate reductase the reduction of fumarate forming succinate.	transcription
55479	7	334970	6	NULL	NULL	0	NULL	ATP citrate lyase			catalyzes					statement 3					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_9_3020_s_23	15838028	2-Oxoglutarate:ferredoxin oxidoreductase catalyzes the carboxylation of succinyl-CoA to 2-oxoglutarate, ATP citrate lyase the ATP-dependent cleavage of citrate to acetyl-CoA and oxaloacetate, and fumarate reductase the reduction of fumarate forming succinate.	transcription
55480	8	334970	6	NULL	NULL	0	NULL	ATP citrate lyase			catalyzes					statement 4					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_9_3020_s_23	15838028	2-Oxoglutarate:ferredoxin oxidoreductase catalyzes the carboxylation of succinyl-CoA to 2-oxoglutarate, ATP citrate lyase the ATP-dependent cleavage of citrate to acetyl-CoA and oxaloacetate, and fumarate reductase the reduction of fumarate forming succinate.	transcription
55481	9	334970	6	NULL	NULL	0	NULL	fumarate			is converted to					succinate					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_9_3020_s_23	15838028	2-Oxoglutarate:ferredoxin oxidoreductase catalyzes the carboxylation of succinyl-CoA to 2-oxoglutarate, ATP citrate lyase the ATP-dependent cleavage of citrate to acetyl-CoA and oxaloacetate, and fumarate reductase the reduction of fumarate forming succinate.	transcription
55482	10	334970	6	NULL	NULL	0	NULL	fumarate reductase			catalyzes					statement 9					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_9_3020_s_23	15838028	2-Oxoglutarate:ferredoxin oxidoreductase catalyzes the carboxylation of succinyl-CoA to 2-oxoglutarate, ATP citrate lyase the ATP-dependent cleavage of citrate to acetyl-CoA and oxaloacetate, and fumarate reductase the reduction of fumarate forming succinate.	transcription
52461	1	334971	5	NULL	NULL	0	NULL	glyoxylate shunt	NULL	functional	regulates	NULL				isocitrate	NULL	levels of			NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_7_3986_s_261	12839772	A functional glyoxylate shunt would regulate isocitrate levels and may reduce intracellular 2-oxoglutarate accumulation by drawing off oxaloacetate via transamination to aspartate.	transcription
52462	2	334971	5	NULL	NULL	0	NULL	glyoxylate shunt	NULL	functional	reduce	NULL				2-oxoglutarate	NULL	accumulation of;;intracellular			NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_7_3986_s_261	12839772	A functional glyoxylate shunt would regulate isocitrate levels and may reduce intracellular 2-oxoglutarate accumulation by drawing off oxaloacetate via transamination to aspartate.	transcription
52463	3	334971	5	NULL	NULL	0	NULL	oxaloacetate	NULL		is transaminated to	NULL				aspartate	NULL				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_7_3986_s_261	12839772	A functional glyoxylate shunt would regulate isocitrate levels and may reduce intracellular 2-oxoglutarate accumulation by drawing off oxaloacetate via transamination to aspartate.	transcription
52464	4	334971	5	NULL	NULL	0	NULL	statement 2	NULL		via	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_7_3986_s_261	12839772	A functional glyoxylate shunt would regulate isocitrate levels and may reduce intracellular 2-oxoglutarate accumulation by drawing off oxaloacetate via transamination to aspartate.	transcription
55508	1	334971	6	NULL	NULL	0	NULL	oxaloacetate			is transaminated to					aspartate					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_7_3986_s_261	12839772	A functional glyoxylate shunt would regulate isocitrate levels and may reduce intracellular 2-oxoglutarate accumulation by drawing off oxaloacetate via transamination to aspartate.	transcription
55509	2	334971	6	NULL	NULL	0	NULL	glyoxylate shunt			regulates					isocitrate 		levels of 			NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_7_3986_s_261	12839772	A functional glyoxylate shunt would regulate isocitrate levels and may reduce intracellular 2-oxoglutarate accumulation by drawing off oxaloacetate via transamination to aspartate.	transcription
52603	1	334972	5	NULL	NULL	0	NULL	HPSOT2 protein	NULL		catalyzes	NULL				oxaloacetate/malate	NULL	transport of			NULL		0	NULL	NULL	NULL	gw60_pnas_99_17_11487_s_185	12177442	Concomitant proteomic identification of two members of the 2-oxoglutarate/malate translocator family (Table  1) suggests that these two proteins may not be differentially expressed spatially or temporally but may differ in substrate specificity: the HPSOT2 protein may catalyze the transport of different dicarboxylic acids (oxaloacetate/malate, malate/glutamate, glutamate/glutamine).	transcription
52604	2	334972	5	NULL	NULL	0	NULL	HPSOT2 protein	NULL		catalyzes	NULL				malate/glutamate	NULL	transport of			NULL		0	NULL	NULL	NULL	gw60_pnas_99_17_11487_s_185	12177442	Concomitant proteomic identification of two members of the 2-oxoglutarate/malate translocator family (Table  1) suggests that these two proteins may not be differentially expressed spatially or temporally but may differ in substrate specificity: the HPSOT2 protein may catalyze the transport of different dicarboxylic acids (oxaloacetate/malate, malate/glutamate, glutamate/glutamine).	transcription
52605	3	334972	5	NULL	NULL	0	NULL	HPSOT2 protein	NULL		catalyzes	NULL				glutamate/glutamine	NULL	transport of			NULL		0	NULL	NULL	NULL	gw60_pnas_99_17_11487_s_185	12177442	Concomitant proteomic identification of two members of the 2-oxoglutarate/malate translocator family (Table  1) suggests that these two proteins may not be differentially expressed spatially or temporally but may differ in substrate specificity: the HPSOT2 protein may catalyze the transport of different dicarboxylic acids (oxaloacetate/malate, malate/glutamate, glutamate/glutamine).	transcription
52606	4	334972	5	NULL	NULL	0	NULL	HPSOT2 protein	NULL		is a member of	NULL				2-oxoglutarate/malate translocator family	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_17_11487_s_185	12177442	Concomitant proteomic identification of two members of the 2-oxoglutarate/malate translocator family (Table  1) suggests that these two proteins may not be differentially expressed spatially or temporally but may differ in substrate specificity: the HPSOT2 protein may catalyze the transport of different dicarboxylic acids (oxaloacetate/malate, malate/glutamate, glutamate/glutamine).	transcription
52607	5	334972	5	NULL	NULL	0	NULL	oxaloacetate/malate	NULL		is a type of	NULL				dicarboxylic acid	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_17_11487_s_185	12177442	Concomitant proteomic identification of two members of the 2-oxoglutarate/malate translocator family (Table  1) suggests that these two proteins may not be differentially expressed spatially or temporally but may differ in substrate specificity: the HPSOT2 protein may catalyze the transport of different dicarboxylic acids (oxaloacetate/malate, malate/glutamate, glutamate/glutamine).	transcription
52608	6	334972	5	NULL	NULL	0	NULL	malate/glutamate	NULL		is a type of	NULL				dicarboxylic acid	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_17_11487_s_185	12177442	Concomitant proteomic identification of two members of the 2-oxoglutarate/malate translocator family (Table  1) suggests that these two proteins may not be differentially expressed spatially or temporally but may differ in substrate specificity: the HPSOT2 protein may catalyze the transport of different dicarboxylic acids (oxaloacetate/malate, malate/glutamate, glutamate/glutamine).	transcription
52609	7	334972	5	NULL	NULL	0	NULL	glutamate/glutamine	NULL		is a type of	NULL				dicarboxylic acids	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_99_17_11487_s_185	12177442	Concomitant proteomic identification of two members of the 2-oxoglutarate/malate translocator family (Table  1) suggests that these two proteins may not be differentially expressed spatially or temporally but may differ in substrate specificity: the HPSOT2 protein may catalyze the transport of different dicarboxylic acids (oxaloacetate/malate, malate/glutamate, glutamate/glutamine).	transcription
55510	1	334972	6	NULL	NULL	0	NULL	HPSOT2 protein			catalyze		may			oxaloacetate/malate		transport of 			NULL		0	NULL	NULL	NULL	gw60_pnas_99_17_11487_s_185	12177442	Concomitant proteomic identification of two members of the 2-oxoglutarate/malate translocator family (Table  1) suggests that these two proteins may not be differentially expressed spatially or temporally but may differ in substrate specificity: the HPSOT2 protein may catalyze the transport of different dicarboxylic acids (oxaloacetate/malate, malate/glutamate, glutamate/glutamine).	transcription
55511	2	334972	6	NULL	NULL	0	NULL	HPSOT2 protein			catalyze		may			malate/glutamate		transport of			NULL		0	NULL	NULL	NULL	gw60_pnas_99_17_11487_s_185	12177442	Concomitant proteomic identification of two members of the 2-oxoglutarate/malate translocator family (Table  1) suggests that these two proteins may not be differentially expressed spatially or temporally but may differ in substrate specificity: the HPSOT2 protein may catalyze the transport of different dicarboxylic acids (oxaloacetate/malate, malate/glutamate, glutamate/glutamine).	transcription
55512	3	334972	6	NULL	NULL	0	NULL	HPSOT2 protein			catalyze		may			glutamate/glutamine		transport of			NULL		0	NULL	NULL	NULL	gw60_pnas_99_17_11487_s_185	12177442	Concomitant proteomic identification of two members of the 2-oxoglutarate/malate translocator family (Table  1) suggests that these two proteins may not be differentially expressed spatially or temporally but may differ in substrate specificity: the HPSOT2 protein may catalyze the transport of different dicarboxylic acids (oxaloacetate/malate, malate/glutamate, glutamate/glutamine).	transcription
52610	1	334973	5	NULL	NULL	0	NULL	homocitrate	NULL		is synthesized from	NULL				2-oxoglutarate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_3_1864_s_215	12427751	It should be noted that we recently found that homocitrate synthase, which catalyzes synthesis of homocitrate from 2-oxoglutarate and acetyl-CoA, the first reaction in lysine biosynthesis of  T. thermophilus HB27, was able to catalyze the synthesis of citrate from oxaloacetate and acetyl-CoA, the corresponding reaction by citrate synthase in the tricarboxylic acid cycle, although homocitrate synthase has no structural similarity to citrate synthase ( ).	transcription
52611	2	334973	5	NULL	NULL	0	NULL	homocitrate	NULL		is synthesized from	NULL				acetyl-CoA	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_3_1864_s_215	12427751	It should be noted that we recently found that homocitrate synthase, which catalyzes synthesis of homocitrate from 2-oxoglutarate and acetyl-CoA, the first reaction in lysine biosynthesis of  T. thermophilus HB27, was able to catalyze the synthesis of citrate from oxaloacetate and acetyl-CoA, the corresponding reaction by citrate synthase in the tricarboxylic acid cycle, although homocitrate synthase has no structural similarity to citrate synthase ( ).	transcription
52612	3	334973	5	NULL	NULL	0	NULL	statement 1	NULL		occurs along with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_3_1864_s_215	12427751	It should be noted that we recently found that homocitrate synthase, which catalyzes synthesis of homocitrate from 2-oxoglutarate and acetyl-CoA, the first reaction in lysine biosynthesis of  T. thermophilus HB27, was able to catalyze the synthesis of citrate from oxaloacetate and acetyl-CoA, the corresponding reaction by citrate synthase in the tricarboxylic acid cycle, although homocitrate synthase has no structural similarity to citrate synthase ( ).	transcription
52613	4	334973	5	NULL	NULL	0	NULL	homocitrate synthase	NULL		catalyzes	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_3_1864_s_215	12427751	It should be noted that we recently found that homocitrate synthase, which catalyzes synthesis of homocitrate from 2-oxoglutarate and acetyl-CoA, the first reaction in lysine biosynthesis of  T. thermophilus HB27, was able to catalyze the synthesis of citrate from oxaloacetate and acetyl-CoA, the corresponding reaction by citrate synthase in the tricarboxylic acid cycle, although homocitrate synthase has no structural similarity to citrate synthase ( ).	transcription
52655	5	334973	5	NULL	NULL	0	NULL	statement 4	NULL		plays a role in	NULL				lysine	NULL	biosynthesis of			NULL	T. thermophilus HB27	0	NULL	NULL	NULL	gw70_jbiolchem_278_3_1864_s_215	12427751	It should be noted that we recently found that homocitrate synthase, which catalyzes synthesis of homocitrate from 2-oxoglutarate and acetyl-CoA, the first reaction in lysine biosynthesis of  T. thermophilus HB27, was able to catalyze the synthesis of citrate from oxaloacetate and acetyl-CoA, the corresponding reaction by citrate synthase in the tricarboxylic acid cycle, although homocitrate synthase has no structural similarity to citrate synthase ( ).	transcription
52656	6	334973	5	NULL	NULL	0	NULL	citrate	NULL		is synthesized from	NULL				oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_3_1864_s_215	12427751	It should be noted that we recently found that homocitrate synthase, which catalyzes synthesis of homocitrate from 2-oxoglutarate and acetyl-CoA, the first reaction in lysine biosynthesis of  T. thermophilus HB27, was able to catalyze the synthesis of citrate from oxaloacetate and acetyl-CoA, the corresponding reaction by citrate synthase in the tricarboxylic acid cycle, although homocitrate synthase has no structural similarity to citrate synthase ( ).	transcription
52657	7	334973	5	NULL	NULL	0	NULL	citrate	NULL		is synthesized from	NULL				acetyl-CoA	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_3_1864_s_215	12427751	It should be noted that we recently found that homocitrate synthase, which catalyzes synthesis of homocitrate from 2-oxoglutarate and acetyl-CoA, the first reaction in lysine biosynthesis of  T. thermophilus HB27, was able to catalyze the synthesis of citrate from oxaloacetate and acetyl-CoA, the corresponding reaction by citrate synthase in the tricarboxylic acid cycle, although homocitrate synthase has no structural similarity to citrate synthase ( ).	transcription
52658	8	334973	5	NULL	NULL	0	NULL	statement 6	NULL		occurs along with	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_3_1864_s_215	12427751	It should be noted that we recently found that homocitrate synthase, which catalyzes synthesis of homocitrate from 2-oxoglutarate and acetyl-CoA, the first reaction in lysine biosynthesis of  T. thermophilus HB27, was able to catalyze the synthesis of citrate from oxaloacetate and acetyl-CoA, the corresponding reaction by citrate synthase in the tricarboxylic acid cycle, although homocitrate synthase has no structural similarity to citrate synthase ( ).	transcription
52659	9	334973	5	NULL	NULL	0	NULL	citrate synthase	NULL		catalyzes	NULL				statement 8	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_3_1864_s_215	12427751	It should be noted that we recently found that homocitrate synthase, which catalyzes synthesis of homocitrate from 2-oxoglutarate and acetyl-CoA, the first reaction in lysine biosynthesis of  T. thermophilus HB27, was able to catalyze the synthesis of citrate from oxaloacetate and acetyl-CoA, the corresponding reaction by citrate synthase in the tricarboxylic acid cycle, although homocitrate synthase has no structural similarity to citrate synthase ( ).	transcription
52660	10	334973	5	NULL	NULL	0	NULL	homocitrate synthase	NULL		catalyzes	NULL				statement 8	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_3_1864_s_215	12427751	It should be noted that we recently found that homocitrate synthase, which catalyzes synthesis of homocitrate from 2-oxoglutarate and acetyl-CoA, the first reaction in lysine biosynthesis of  T. thermophilus HB27, was able to catalyze the synthesis of citrate from oxaloacetate and acetyl-CoA, the corresponding reaction by citrate synthase in the tricarboxylic acid cycle, although homocitrate synthase has no structural similarity to citrate synthase ( ).	transcription
52661	11	334973	5	NULL	NULL	0	NULL	homocitrate synthase	NULL		is not similar to	NULL	structurally			citrate synthase	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_3_1864_s_215	12427751	It should be noted that we recently found that homocitrate synthase, which catalyzes synthesis of homocitrate from 2-oxoglutarate and acetyl-CoA, the first reaction in lysine biosynthesis of  T. thermophilus HB27, was able to catalyze the synthesis of citrate from oxaloacetate and acetyl-CoA, the corresponding reaction by citrate synthase in the tricarboxylic acid cycle, although homocitrate synthase has no structural similarity to citrate synthase ( ).	transcription
55513	1	334973	6	NULL	NULL	0	NULL	2-oxoglutarate			synthesizes					homocitrate					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_3_1864_s_215	12427751	It should be noted that we recently found that homocitrate synthase, which catalyzes synthesis of homocitrate from 2-oxoglutarate and acetyl-CoA, the first reaction in lysine biosynthesis of  T. thermophilus HB27, was able to catalyze the synthesis of citrate from oxaloacetate and acetyl-CoA, the corresponding reaction by citrate synthase in the tricarboxylic acid cycle, although homocitrate synthase has no structural similarity to citrate synthase ( ).	transcription
55515	2	334973	6	NULL	NULL	0	NULL	acetyl-CoA			synthesizes					homocitrate					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_3_1864_s_215	12427751	It should be noted that we recently found that homocitrate synthase, which catalyzes synthesis of homocitrate from 2-oxoglutarate and acetyl-CoA, the first reaction in lysine biosynthesis of  T. thermophilus HB27, was able to catalyze the synthesis of citrate from oxaloacetate and acetyl-CoA, the corresponding reaction by citrate synthase in the tricarboxylic acid cycle, although homocitrate synthase has no structural similarity to citrate synthase ( ).	transcription
55516	3	334973	6	NULL	NULL	0	NULL	statement 1			occurs simultaneously with					statement 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_3_1864_s_215	12427751	It should be noted that we recently found that homocitrate synthase, which catalyzes synthesis of homocitrate from 2-oxoglutarate and acetyl-CoA, the first reaction in lysine biosynthesis of  T. thermophilus HB27, was able to catalyze the synthesis of citrate from oxaloacetate and acetyl-CoA, the corresponding reaction by citrate synthase in the tricarboxylic acid cycle, although homocitrate synthase has no structural similarity to citrate synthase ( ).	transcription
55517	4	334973	6	NULL	NULL	0	NULL	homocitrate synthase			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_3_1864_s_215	12427751	It should be noted that we recently found that homocitrate synthase, which catalyzes synthesis of homocitrate from 2-oxoglutarate and acetyl-CoA, the first reaction in lysine biosynthesis of  T. thermophilus HB27, was able to catalyze the synthesis of citrate from oxaloacetate and acetyl-CoA, the corresponding reaction by citrate synthase in the tricarboxylic acid cycle, although homocitrate synthase has no structural similarity to citrate synthase ( ).	transcription
55518	5	334973	6	NULL	NULL	0	NULL	homocitrate synthase			catalyzes					statement 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_3_1864_s_215	12427751	It should be noted that we recently found that homocitrate synthase, which catalyzes synthesis of homocitrate from 2-oxoglutarate and acetyl-CoA, the first reaction in lysine biosynthesis of  T. thermophilus HB27, was able to catalyze the synthesis of citrate from oxaloacetate and acetyl-CoA, the corresponding reaction by citrate synthase in the tricarboxylic acid cycle, although homocitrate synthase has no structural similarity to citrate synthase ( ).	transcription
55519	6	334973	6	NULL	NULL	0	NULL	statement 3			occurs during					lysine		biosynthesis of			NULL	T. thermophilus HB27	0	NULL	NULL	NULL	gw70_jbiolchem_278_3_1864_s_215	12427751	It should be noted that we recently found that homocitrate synthase, which catalyzes synthesis of homocitrate from 2-oxoglutarate and acetyl-CoA, the first reaction in lysine biosynthesis of  T. thermophilus HB27, was able to catalyze the synthesis of citrate from oxaloacetate and acetyl-CoA, the corresponding reaction by citrate synthase in the tricarboxylic acid cycle, although homocitrate synthase has no structural similarity to citrate synthase ( ).	transcription
55520	7	334973	6	NULL	NULL	0	NULL	oxaloacetate			synthesizes					citrate					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_3_1864_s_215	12427751	It should be noted that we recently found that homocitrate synthase, which catalyzes synthesis of homocitrate from 2-oxoglutarate and acetyl-CoA, the first reaction in lysine biosynthesis of  T. thermophilus HB27, was able to catalyze the synthesis of citrate from oxaloacetate and acetyl-CoA, the corresponding reaction by citrate synthase in the tricarboxylic acid cycle, although homocitrate synthase has no structural similarity to citrate synthase ( ).	transcription
55554	8	334973	6	NULL	NULL	0	NULL	acetyl-CoA			synthesizes					citrate					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_3_1864_s_215	12427751	It should be noted that we recently found that homocitrate synthase, which catalyzes synthesis of homocitrate from 2-oxoglutarate and acetyl-CoA, the first reaction in lysine biosynthesis of  T. thermophilus HB27, was able to catalyze the synthesis of citrate from oxaloacetate and acetyl-CoA, the corresponding reaction by citrate synthase in the tricarboxylic acid cycle, although homocitrate synthase has no structural similarity to citrate synthase ( ).	transcription
55555	9	334973	6	NULL	NULL	0	NULL	statement 7			occurs simultaneously with					statement 8					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_3_1864_s_215	12427751	It should be noted that we recently found that homocitrate synthase, which catalyzes synthesis of homocitrate from 2-oxoglutarate and acetyl-CoA, the first reaction in lysine biosynthesis of  T. thermophilus HB27, was able to catalyze the synthesis of citrate from oxaloacetate and acetyl-CoA, the corresponding reaction by citrate synthase in the tricarboxylic acid cycle, although homocitrate synthase has no structural similarity to citrate synthase ( ).	transcription
55556	10	334973	6	NULL	NULL	0	NULL	homocitrate synthase			catalyzes					statement 7					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_3_1864_s_215	12427751	It should be noted that we recently found that homocitrate synthase, which catalyzes synthesis of homocitrate from 2-oxoglutarate and acetyl-CoA, the first reaction in lysine biosynthesis of  T. thermophilus HB27, was able to catalyze the synthesis of citrate from oxaloacetate and acetyl-CoA, the corresponding reaction by citrate synthase in the tricarboxylic acid cycle, although homocitrate synthase has no structural similarity to citrate synthase ( ).	transcription
55557	11	334973	6	NULL	NULL	0	NULL	homocitrate synthase			catalyzes					statement 8					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_3_1864_s_215	12427751	It should be noted that we recently found that homocitrate synthase, which catalyzes synthesis of homocitrate from 2-oxoglutarate and acetyl-CoA, the first reaction in lysine biosynthesis of  T. thermophilus HB27, was able to catalyze the synthesis of citrate from oxaloacetate and acetyl-CoA, the corresponding reaction by citrate synthase in the tricarboxylic acid cycle, although homocitrate synthase has no structural similarity to citrate synthase ( ).	transcription
55558	12	334973	6	NULL	NULL	0	NULL	homocitrate synthase			is dissimilar to		structurally			citrate synthase					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_3_1864_s_215	12427751	It should be noted that we recently found that homocitrate synthase, which catalyzes synthesis of homocitrate from 2-oxoglutarate and acetyl-CoA, the first reaction in lysine biosynthesis of  T. thermophilus HB27, was able to catalyze the synthesis of citrate from oxaloacetate and acetyl-CoA, the corresponding reaction by citrate synthase in the tricarboxylic acid cycle, although homocitrate synthase has no structural similarity to citrate synthase ( ).	transcription
52662	1	334974	5	NULL	NULL	0	NULL	oxaloacetate	NULL		is converted to	NULL				phosphoenolpyruvate	NULL				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_309_1_328_s_28	14722324	Phosphoenolpyruvate carboxykinase catalyzes the conversion of oxaloacetate to phosphoenolpyruvate, the rate-limiting step in gluconeogenesis.	transcription
52663	2	334974	5	NULL	NULL	0	NULL	Phosphoenolpyruvate carboxykinase			catalyzes					rate-limiting step					NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_309_1_328_s_28	14722324	Phosphoenolpyruvate carboxykinase catalyzes the conversion of oxaloacetate to phosphoenolpyruvate, the rate-limiting step in gluconeogenesis.	transcription
52664	3	334974	5	NULL	NULL	0	NULL	statement 2			conversion of		for			statement 1					NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_309_1_328_s_28	14722324	Phosphoenolpyruvate carboxykinase catalyzes the conversion of oxaloacetate to phosphoenolpyruvate, the rate-limiting step in gluconeogenesis.	transcription
54319	4	334974	5	NULL	NULL	0	NULL	statement 1			occurs in					gluconeogenesis					NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_309_1_328_s_28	14722324	Phosphoenolpyruvate carboxykinase catalyzes the conversion of oxaloacetate to phosphoenolpyruvate, the rate-limiting step in gluconeogenesis.	transcription
55559	1	334974	6	NULL	NULL	0	NULL	oxaloacetate			is converted to					phosphoenolpyruvate					NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_309_1_328_s_28	14722324	Phosphoenolpyruvate carboxykinase catalyzes the conversion of oxaloacetate to phosphoenolpyruvate, the rate-limiting step in gluconeogenesis.	transcription
55560	2	334974	6	NULL	NULL	0	NULL	Phosphoenolpyruvate carboxykinase			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_309_1_328_s_28	14722324	Phosphoenolpyruvate carboxykinase catalyzes the conversion of oxaloacetate to phosphoenolpyruvate, the rate-limiting step in gluconeogenesis.	transcription
55561	3	334974	6	NULL	NULL	0	NULL	statement 1			is an important step in					gluconeogenesis					NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_309_1_328_s_28	14722324	Phosphoenolpyruvate carboxykinase catalyzes the conversion of oxaloacetate to phosphoenolpyruvate, the rate-limiting step in gluconeogenesis.	transcription
52665	1	334975	5	NULL	NULL	0	NULL	oxaloacetate	NULL		is converted to	NULL				phosphoenolpyruvate	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1454_2_133_s_102	10381558	Phosphoenolpyruvate carboxykinase catalyzes the conversion of oxaloacetate to phosphoenolpyruvate which is then utilized by the gluconeogenic pathway.	transcription
52666	2	334975	5	NULL	NULL	0	NULL	Phosphoenolpyruvate carboxykinase	NULL		catalyzes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1454_2_133_s_102	10381558	Phosphoenolpyruvate carboxykinase catalyzes the conversion of oxaloacetate to phosphoenolpyruvate which is then utilized by the gluconeogenic pathway.	transcription
52667	3	334975	5	NULL	NULL	0	NULL	phosphoenolpyruvate	NULL		is utilized by	NULL				gluconeogenic pathway	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1454_2_133_s_102	10381558	Phosphoenolpyruvate carboxykinase catalyzes the conversion of oxaloacetate to phosphoenolpyruvate which is then utilized by the gluconeogenic pathway.	transcription
55562	1	334975	6	NULL	NULL	0	NULL	oxaloacetate			is converted to					phosphoenolpyruvate					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1454_2_133_s_102	10381558	Phosphoenolpyruvate carboxykinase catalyzes the conversion of oxaloacetate to phosphoenolpyruvate which is then utilized by the gluconeogenic pathway.	transcription
55563	2	334975	6	NULL	NULL	0	NULL	Phosphoenolpyruvate carboxykinase			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1454_2_133_s_102	10381558	Phosphoenolpyruvate carboxykinase catalyzes the conversion of oxaloacetate to phosphoenolpyruvate which is then utilized by the gluconeogenic pathway.	transcription
55564	3	334975	6	NULL	NULL	0	NULL	Phosphoenolpyruvate			is utilized by					gluconeogenic pathway					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1454_2_133_s_102	10381558	Phosphoenolpyruvate carboxykinase catalyzes the conversion of oxaloacetate to phosphoenolpyruvate which is then utilized by the gluconeogenic pathway.	transcription
52668	1	334976	5	NULL	NULL	0	NULL	oxaloacetate	NULL		is converted to	NULL				phosphoenolpyruvate	NULL				NULL		0	NULL	NULL	NULL	gw60_diabetes_51_3_624_s_17	11872659	A regulatory step of this pathway is the conversion of oxaloacetate to phosphoenolpyruvate catalyzed by PEPCK ( 2).	transcription
52669	2	334976	5	NULL	NULL	0	NULL	PEPCK	NULL		catalyzes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_diabetes_51_3_624_s_17	11872659	A regulatory step of this pathway is the conversion of oxaloacetate to phosphoenolpyruvate catalyzed by PEPCK ( 2).	transcription
55565	1	334976	6	NULL	NULL	0	NULL	oxaloacetate			is converted to					phosphoenolpyruvate					NULL		0	NULL	NULL	NULL	gw60_diabetes_51_3_624_s_17	11872659	A regulatory step of this pathway is the conversion of oxaloacetate to phosphoenolpyruvate catalyzed by PEPCK ( 2).	transcription
55566	2	334976	6	NULL	NULL	0	NULL	PEPCK			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw60_diabetes_51_3_624_s_17	11872659	A regulatory step of this pathway is the conversion of oxaloacetate to phosphoenolpyruvate catalyzed by PEPCK ( 2).	transcription
52670	1	334977	5	NULL	NULL	0	NULL	oxaloacetate	NULL		is converted to	NULL				phosphoenolpyruvate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_5_3446_s_37	10652338	PEPCK catalyzes the conversion of oxaloacetate to phosphoenolpyruvate, a rate-controlling step in hepatic gluconeogenesis.	transcription
52671	2	334977	5	NULL	NULL	0	NULL	PEPCK	NULL		catalyzes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_5_3446_s_37	10652338	PEPCK catalyzes the conversion of oxaloacetate to phosphoenolpyruvate, a rate-controlling step in hepatic gluconeogenesis.	transcription
52672	3	334977	5	NULL	NULL	0	NULL	statement 1	NULL		is a type of	NULL				rate-controlling step in hepatic gluconeogenesis	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_5_3446_s_37	10652338	PEPCK catalyzes the conversion of oxaloacetate to phosphoenolpyruvate, a rate-controlling step in hepatic gluconeogenesis.	transcription
52673	1	334978	5	NULL	NULL	0	NULL	PEPCK	NULL		is	NULL				phosphoenolpyruvate carboxykinase	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_31_28272_s_13	15951444	Phosphoenolpyruvate carboxykinase (PEPCK)  1 catalyzes the conversion of oxaloacetate to phosphoenolpyruvate, a rate-limiting step in gluconeogenesis.	transcription
52674	2	334978	5	NULL	NULL	0	NULL	oxaloacetate	NULL		is converted to	NULL				phosphoenolpyruvate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_31_28272_s_13	15951444	Phosphoenolpyruvate carboxykinase (PEPCK)  1 catalyzes the conversion of oxaloacetate to phosphoenolpyruvate, a rate-limiting step in gluconeogenesis.	transcription
52675	3	334978	5	NULL	NULL	0	NULL	PEPCK	NULL		catalyzes	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_31_28272_s_13	15951444	Phosphoenolpyruvate carboxykinase (PEPCK)  1 catalyzes the conversion of oxaloacetate to phosphoenolpyruvate, a rate-limiting step in gluconeogenesis.	transcription
52676	4	334978	5	NULL	NULL	0	NULL	statement 2	NULL		is a type of	NULL				rate-limiting step in gluconeogenesis	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_31_28272_s_13	15951444	Phosphoenolpyruvate carboxykinase (PEPCK)  1 catalyzes the conversion of oxaloacetate to phosphoenolpyruvate, a rate-limiting step in gluconeogenesis.	transcription
55569	1	334978	6	NULL	NULL	0	NULL	PEPCK			is					Phosphoenolpyruvate carboxykinase					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_31_28272_s_13	15951444	Phosphoenolpyruvate carboxykinase (PEPCK)  1 catalyzes the conversion of oxaloacetate to phosphoenolpyruvate, a rate-limiting step in gluconeogenesis.	transcription
55570	2	334978	6	NULL	NULL	0	NULL	oxaloacetate			is converted to					phosphoenolpyruvate					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_31_28272_s_13	15951444	Phosphoenolpyruvate carboxykinase (PEPCK)  1 catalyzes the conversion of oxaloacetate to phosphoenolpyruvate, a rate-limiting step in gluconeogenesis.	transcription
55571	3	334978	6	NULL	NULL	0	NULL	PEPCK			catalyzes					statement  2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_31_28272_s_13	15951444	Phosphoenolpyruvate carboxykinase (PEPCK)  1 catalyzes the conversion of oxaloacetate to phosphoenolpyruvate, a rate-limiting step in gluconeogenesis.	transcription
55572	4	334978	6	NULL	NULL	0	NULL	statement 1			is a step in					gluconeogenesis					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_31_28272_s_13	15951444	Phosphoenolpyruvate carboxykinase (PEPCK)  1 catalyzes the conversion of oxaloacetate to phosphoenolpyruvate, a rate-limiting step in gluconeogenesis.	transcription
52677	1	334979	5	NULL	NULL	0	NULL	oxaloacetate	NULL		is converted to	NULL				phosphoenolpyruvate	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_17_6508_s_11	10938127	A key step in gluconeogenesis is the formation of phosphoenolpyruvate from oxaloacetate, which is catalyzed by phosphoenolpyruvate carboxykinase (PEPCK).	transcription
52678	2	334979	5	NULL	NULL	0	NULL	statement 1	NULL		is a key step in	NULL				gluconeogenesis	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_17_6508_s_11	10938127	A key step in gluconeogenesis is the formation of phosphoenolpyruvate from oxaloacetate, which is catalyzed by phosphoenolpyruvate carboxykinase (PEPCK).	transcription
52679	3	334979	5	NULL	NULL	0	NULL	PEPCK	NULL		catalyzes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_17_6508_s_11	10938127	A key step in gluconeogenesis is the formation of phosphoenolpyruvate from oxaloacetate, which is catalyzed by phosphoenolpyruvate carboxykinase (PEPCK).	transcription
52680	4	334979	5	NULL	NULL	0	NULL	PEPCK	NULL		is	NULL				phosphoenolpyruvate carboxykinase	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_17_6508_s_11	10938127	A key step in gluconeogenesis is the formation of phosphoenolpyruvate from oxaloacetate, which is catalyzed by phosphoenolpyruvate carboxykinase (PEPCK).	transcription
52681	1	334980	5	NULL	NULL	0	NULL	PEP	NULL		is	NULL				phosphoenolpyruvate	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1546_1_242_s_4	11257527	1.31) catalyzes the essentially irreversible formation of oxaloacetate and inorganic phosphate from phosphoenolpyruvate (PEP) and bicarbonate, in the presence of Mg2+ [  1.	transcription
52682	2	334980	5	NULL	NULL	0	NULL	PEP			forms		irreversibly			oxaloacetate					NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1546_1_242_s_4	11257527	1.31) catalyzes the essentially irreversible formation of oxaloacetate and inorganic phosphate from phosphoenolpyruvate (PEP) and bicarbonate, in the presence of Mg2+ [  1.	transcription
52683	3	334980	5	NULL	NULL	0	NULL	bicarbonate			forms		irreversibly			oxaloacetate					NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1546_1_242_s_4	11257527	1.31) catalyzes the essentially irreversible formation of oxaloacetate and inorganic phosphate from phosphoenolpyruvate (PEP) and bicarbonate, in the presence of Mg2+ [  1.	transcription
58483	4	334980	5	NULL	NULL	0	NULL	statement 2			occurs simultaneously with					statement 3					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1546_1_242_s_4	11257527	1.31) catalyzes the essentially irreversible formation of oxaloacetate and inorganic phosphate from phosphoenolpyruvate (PEP) and bicarbonate, in the presence of Mg2+ [  1.	transcription
58484	5	334980	5	NULL	NULL	0	NULL	PEP			forms		irreversibly			inorganic phosphate					NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1546_1_242_s_4	11257527	1.31) catalyzes the essentially irreversible formation of oxaloacetate and inorganic phosphate from phosphoenolpyruvate (PEP) and bicarbonate, in the presence of Mg2+ [  1.	transcription
58485	6	334980	5	NULL	NULL	0	NULL	bicarbonate			forms		irreversibly			inorganic phosphate					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1546_1_242_s_4	11257527	1.31) catalyzes the essentially irreversible formation of oxaloacetate and inorganic phosphate from phosphoenolpyruvate (PEP) and bicarbonate, in the presence of Mg2+ [  1.	transcription
58486	7	334980	5	NULL	NULL	0	NULL	statement 5			occurs simultaneously with					statement 6					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1546_1_242_s_4	11257527	1.31) catalyzes the essentially irreversible formation of oxaloacetate and inorganic phosphate from phosphoenolpyruvate (PEP) and bicarbonate, in the presence of Mg2+ [  1.	transcription
58487	8	334980	5	NULL	NULL	0	NULL	statement 4			in the presence of					Mg2+					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1546_1_242_s_4	11257527	1.31) catalyzes the essentially irreversible formation of oxaloacetate and inorganic phosphate from phosphoenolpyruvate (PEP) and bicarbonate, in the presence of Mg2+ [  1.	transcription
58488	9	334980	5	NULL	NULL	0	NULL	statement 7			in the presence of					Mg2+					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1546_1_242_s_4	11257527	1.31) catalyzes the essentially irreversible formation of oxaloacetate and inorganic phosphate from phosphoenolpyruvate (PEP) and bicarbonate, in the presence of Mg2+ [  1.	transcription
55576	1	334980	6	NULL	NULL	0	NULL	PEP			forms					oxaloacetate					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1546_1_242_s_4	11257527	1.31) catalyzes the essentially irreversible formation of oxaloacetate and inorganic phosphate from phosphoenolpyruvate (PEP) and bicarbonate, in the presence of Mg2+ [  1.	transcription
55577	2	334980	6	NULL	NULL	0	NULL	PEP			is					phosphoenolpyruvate					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1546_1_242_s_4	11257527	1.31) catalyzes the essentially irreversible formation of oxaloacetate and inorganic phosphate from phosphoenolpyruvate (PEP) and bicarbonate, in the presence of Mg2+ [  1.	transcription
55578	3	334980	6	NULL	NULL	0	NULL	bicarbonate			forms					oxaloacetate					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1546_1_242_s_4	11257527	1.31) catalyzes the essentially irreversible formation of oxaloacetate and inorganic phosphate from phosphoenolpyruvate (PEP) and bicarbonate, in the presence of Mg2+ [  1.	transcription
55579	4	334980	6	NULL	NULL	0	NULL	statement 1			occurs in the presence of					Mg2+					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1546_1_242_s_4	11257527	1.31) catalyzes the essentially irreversible formation of oxaloacetate and inorganic phosphate from phosphoenolpyruvate (PEP) and bicarbonate, in the presence of Mg2+ [  1.	transcription
55580	5	334980	6	NULL	NULL	0	NULL	statement 3			occurs in the presence of					Mg2+					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1546_1_242_s_4	11257527	1.31) catalyzes the essentially irreversible formation of oxaloacetate and inorganic phosphate from phosphoenolpyruvate (PEP) and bicarbonate, in the presence of Mg2+ [  1.	transcription
52684	1	334981	5	NULL	NULL	0	NULL	HCO3	NULL		is fixed to	NULL				phosphoenolpyruvate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_36_27917_s_11	10871630	1.31; PEPC)1 catalyzes the fixation of HCO3  to the receptor phosphoenolpyruvate resulting in the formation of oxaloacetate and inorganic phosphate.	transcription
52685	2	334981	5	NULL	NULL	0	NULL	phosphoenolpyruvate	NULL		is a type of	NULL				receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_36_27917_s_11	10871630	1.31; PEPC)1 catalyzes the fixation of HCO3  to the receptor phosphoenolpyruvate resulting in the formation of oxaloacetate and inorganic phosphate.	transcription
52686	3	334981	5	NULL	NULL	0	NULL	PEPC	NULL		catalyzes	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_36_27917_s_11	10871630	1.31; PEPC)1 catalyzes the fixation of HCO3  to the receptor phosphoenolpyruvate resulting in the formation of oxaloacetate and inorganic phosphate.	transcription
52687	4	334981	5	NULL	NULL	0	NULL	statement 3	NULL		results in	NULL				oxaloacetate	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_36_27917_s_11	10871630	1.31; PEPC)1 catalyzes the fixation of HCO3  to the receptor phosphoenolpyruvate resulting in the formation of oxaloacetate and inorganic phosphate.	transcription
52688	5	334981	5	NULL	NULL	0	NULL	statement 3	NULL		results in	NULL				inorganic phosphate	NULL	formation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_36_27917_s_11	10871630	1.31; PEPC)1 catalyzes the fixation of HCO3  to the receptor phosphoenolpyruvate resulting in the formation of oxaloacetate and inorganic phosphate.	transcription
52689	6	334981	5	NULL	NULL	0	NULL	statement 4	NULL		occurs along with	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_36_27917_s_11	10871630	1.31; PEPC)1 catalyzes the fixation of HCO3  to the receptor phosphoenolpyruvate resulting in the formation of oxaloacetate and inorganic phosphate.	transcription
55581	1	334981	6	NULL	NULL	0	NULL	HCO3			fixes					phosphoenolpyruvate receptor					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_36_27917_s_11	10871630	1.31; PEPC)1 catalyzes the fixation of HCO3  to the receptor phosphoenolpyruvate resulting in the formation of oxaloacetate and inorganic phosphate.	transcription
55582	2	334981	6	NULL	NULL	0	NULL	PEPC1			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_36_27917_s_11	10871630	1.31; PEPC)1 catalyzes the fixation of HCO3  to the receptor phosphoenolpyruvate resulting in the formation of oxaloacetate and inorganic phosphate.	transcription
55583	3	334981	6	NULL	NULL	0	NULL	statement 1			results in 					oxaloacetate		formation of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_36_27917_s_11	10871630	1.31; PEPC)1 catalyzes the fixation of HCO3  to the receptor phosphoenolpyruvate resulting in the formation of oxaloacetate and inorganic phosphate.	transcription
55584	4	334981	6	NULL	NULL	0	NULL	statement 1			results in					inorganic phosphate		formation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_36_27917_s_11	10871630	1.31; PEPC)1 catalyzes the fixation of HCO3  to the receptor phosphoenolpyruvate resulting in the formation of oxaloacetate and inorganic phosphate.	transcription
58489	1	334983	5	NULL	NULL	0	NULL	C4-decarboxylating backflux			occurs from					TCA cycle					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_12_5843_s_265	12450803	It is known that  C. glutamicum has several enzymes, such as phosphoenolpyruvate carboxykinase and oxaloacetate decarboxylase, that catalyze a C4-decarboxylating backflux from the TCA cycle to glycolysis ( 14).	transcription
58490	2	334983	5	NULL	NULL	0	NULL	C4-decarboxylating backflux			to					glycolysis					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_12_5843_s_265	12450803	It is known that  C. glutamicum has several enzymes, such as phosphoenolpyruvate carboxykinase and oxaloacetate decarboxylase, that catalyze a C4-decarboxylating backflux from the TCA cycle to glycolysis ( 14).	transcription
58491	3	334983	5	NULL	NULL	0	NULL	statement 1			occurs along with					statement 2					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_12_5843_s_265	12450803	It is known that  C. glutamicum has several enzymes, such as phosphoenolpyruvate carboxykinase and oxaloacetate decarboxylase, that catalyze a C4-decarboxylating backflux from the TCA cycle to glycolysis ( 14).	transcription
58492	4	334983	5	NULL	NULL	0	NULL	phosphoenolpyruvate carboxykinase		C. glutamicum	catalyzes					statement 3					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_12_5843_s_265	12450803	It is known that  C. glutamicum has several enzymes, such as phosphoenolpyruvate carboxykinase and oxaloacetate decarboxylase, that catalyze a C4-decarboxylating backflux from the TCA cycle to glycolysis ( 14).	transcription
58493	5	334983	5	NULL	NULL	0	NULL	oxaloacetate decarboxylase		C. glutamicum	catalyzes					statement 3					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_12_5843_s_265	12450803	It is known that  C. glutamicum has several enzymes, such as phosphoenolpyruvate carboxykinase and oxaloacetate decarboxylase, that catalyze a C4-decarboxylating backflux from the TCA cycle to glycolysis ( 14).	transcription
55585	1	334983	6	NULL	NULL	0	NULL	phosphoenolpyruvate carboxykinase			catalyze					C4-decarboxylating backflux					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_12_5843_s_265	12450803	It is known that  C. glutamicum has several enzymes, such as phosphoenolpyruvate carboxykinase and oxaloacetate decarboxylase, that catalyze a C4-decarboxylating backflux from the TCA cycle to glycolysis ( 14).	transcription
55586	2	334983	6	NULL	NULL	0	NULL	statement 1			occurs from					TCA cycle					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_12_5843_s_265	12450803	It is known that  C. glutamicum has several enzymes, such as phosphoenolpyruvate carboxykinase and oxaloacetate decarboxylase, that catalyze a C4-decarboxylating backflux from the TCA cycle to glycolysis ( 14).	transcription
55587	3	334983	6	NULL	NULL	0	NULL	statement 1			occurs to					glycolysis					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_12_5843_s_265	12450803	It is known that  C. glutamicum has several enzymes, such as phosphoenolpyruvate carboxykinase and oxaloacetate decarboxylase, that catalyze a C4-decarboxylating backflux from the TCA cycle to glycolysis ( 14).	transcription
55588	4	334983	6	NULL	NULL	0	NULL	oxaloacetate decarboxylase			catalyze					C4-decarboxylating backflux					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_12_5843_s_265	12450803	It is known that  C. glutamicum has several enzymes, such as phosphoenolpyruvate carboxykinase and oxaloacetate decarboxylase, that catalyze a C4-decarboxylating backflux from the TCA cycle to glycolysis ( 14).	transcription
52690	1	334984	5	NULL	NULL	0	NULL	PEP	NULL		is	NULL				phosphoenolpyruvate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_25_17238_s_14	16624802	It catalyzes the irreversible, biotin-independent carboxylation of phosphoenolpyruvate (PEP) in the presence of   and Mg2+ (or Mn2+) to yield Pi and oxaloacetate and, thus, is involved intimately in photosynthetic and/or anaplerotic C4 dicarboxylic acid metabolism in these organisms.	transcription
52691	2	334984	5	NULL	NULL	0	NULL	PEP	NULL		undergoes	NULL				carboxylation	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_25_17238_s_14	16624802	It catalyzes the irreversible, biotin-independent carboxylation of phosphoenolpyruvate (PEP) in the presence of   and Mg2+ (or Mn2+) to yield Pi and oxaloacetate and, thus, is involved intimately in photosynthetic and/or anaplerotic C4 dicarboxylic acid metabolism in these organisms.	transcription
52692	3	334984	5	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				biotin	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_25_17238_s_14	16624802	It catalyzes the irreversible, biotin-independent carboxylation of phosphoenolpyruvate (PEP) in the presence of   and Mg2+ (or Mn2+) to yield Pi and oxaloacetate and, thus, is involved intimately in photosynthetic and/or anaplerotic C4 dicarboxylic acid metabolism in these organisms.	transcription
52693	4	334984	5	NULL	NULL	0	NULL	statement 2	NULL		in the presence of	NULL				Mg2+	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_25_17238_s_14	16624802	It catalyzes the irreversible, biotin-independent carboxylation of phosphoenolpyruvate (PEP) in the presence of   and Mg2+ (or Mn2+) to yield Pi and oxaloacetate and, thus, is involved intimately in photosynthetic and/or anaplerotic C4 dicarboxylic acid metabolism in these organisms.	transcription
52694	5	334984	5	NULL	NULL	0	NULL	statement 2	NULL		in the presence of	NULL				Mn2+	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_25_17238_s_14	16624802	It catalyzes the irreversible, biotin-independent carboxylation of phosphoenolpyruvate (PEP) in the presence of   and Mg2+ (or Mn2+) to yield Pi and oxaloacetate and, thus, is involved intimately in photosynthetic and/or anaplerotic C4 dicarboxylic acid metabolism in these organisms.	transcription
52695	6	334984	5	NULL	NULL	0	NULL	statement 4	NULL		is an alternative to	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_25_17238_s_14	16624802	It catalyzes the irreversible, biotin-independent carboxylation of phosphoenolpyruvate (PEP) in the presence of   and Mg2+ (or Mn2+) to yield Pi and oxaloacetate and, thus, is involved intimately in photosynthetic and/or anaplerotic C4 dicarboxylic acid metabolism in these organisms.	transcription
52696	7	334984	5	NULL	NULL	0	NULL	statement 2	NULL		yields	NULL				oxaloacetate	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_25_17238_s_14	16624802	It catalyzes the irreversible, biotin-independent carboxylation of phosphoenolpyruvate (PEP) in the presence of   and Mg2+ (or Mn2+) to yield Pi and oxaloacetate and, thus, is involved intimately in photosynthetic and/or anaplerotic C4 dicarboxylic acid metabolism in these organisms.	transcription
52697	8	334984	5	NULL	NULL	0	NULL	statement 2	NULL		yields	NULL				Pi	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_25_17238_s_14	16624802	It catalyzes the irreversible, biotin-independent carboxylation of phosphoenolpyruvate (PEP) in the presence of   and Mg2+ (or Mn2+) to yield Pi and oxaloacetate and, thus, is involved intimately in photosynthetic and/or anaplerotic C4 dicarboxylic acid metabolism in these organisms.	transcription
52698	9	334984	5	NULL	NULL	0	NULL	statement 7	NULL		occurs along with	NULL				statement 8	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_25_17238_s_14	16624802	It catalyzes the irreversible, biotin-independent carboxylation of phosphoenolpyruvate (PEP) in the presence of   and Mg2+ (or Mn2+) to yield Pi and oxaloacetate and, thus, is involved intimately in photosynthetic and/or anaplerotic C4 dicarboxylic acid metabolism in these organisms.	transcription
52699	10	334984	5	NULL	NULL	0	NULL	statement 2	NULL		is involved in	NULL	intimately			photosynthetic C4 dicarboxylic acid metabolism	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_25_17238_s_14	16624802	It catalyzes the irreversible, biotin-independent carboxylation of phosphoenolpyruvate (PEP) in the presence of   and Mg2+ (or Mn2+) to yield Pi and oxaloacetate and, thus, is involved intimately in photosynthetic and/or anaplerotic C4 dicarboxylic acid metabolism in these organisms.	transcription
52700	11	334984	5	NULL	NULL	0	NULL	statement 2	NULL		is involved in	NULL	intimately			anaplerotic C4 dicarboxylic acid metabolism	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_25_17238_s_14	16624802	It catalyzes the irreversible, biotin-independent carboxylation of phosphoenolpyruvate (PEP) in the presence of   and Mg2+ (or Mn2+) to yield Pi and oxaloacetate and, thus, is involved intimately in photosynthetic and/or anaplerotic C4 dicarboxylic acid metabolism in these organisms.	transcription
55589	1	334985	6	NULL	NULL	0	NULL	PEP			forms		reversibly			oxaloacetate					NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_biochimie_88_6_16469427_s_2	16469427	Saccharomyces cerevisiae phosphoenolpyruvate (PEP) carboxykinase catalyzes  the reversible formation of oxaloacetate and adenosine triphosphate from  PEP, adenosine diphosphate and carbon dioxide, and uses Mn(2+) as the  activating metal ion.	transcription
55590	2	334985	6	NULL	NULL	0	NULL	PEP			forms		reversibly			adenosine triphosphate					NULL		NULL	NULL	NULL	NULL	abs-batch0740-0759_biochimie_88_6_16469427_s_2	16469427	Saccharomyces cerevisiae phosphoenolpyruvate (PEP) carboxykinase catalyzes  the reversible formation of oxaloacetate and adenosine triphosphate from  PEP, adenosine diphosphate and carbon dioxide, and uses Mn(2+) as the  activating metal ion.	transcription
55591	3	334985	6	NULL	NULL	0	NULL	PEP carboxykinase 			catalyzes					statement 1					NULL	Saccharomyces cerevisiae	0	NULL	NULL	NULL	abs-batch0740-0759_biochimie_88_6_16469427_s_2	16469427	Saccharomyces cerevisiae phosphoenolpyruvate (PEP) carboxykinase catalyzes  the reversible formation of oxaloacetate and adenosine triphosphate from  PEP, adenosine diphosphate and carbon dioxide, and uses Mn(2+) as the  activating metal ion.	transcription
55592	4	334985	6	NULL	NULL	0	NULL	PEP carboxykinase			catalyzes					statement 2					NULL	Saccharomyces cerevisiae	NULL	NULL	NULL	NULL	abs-batch0740-0759_biochimie_88_6_16469427_s_2	16469427	Saccharomyces cerevisiae phosphoenolpyruvate (PEP) carboxykinase catalyzes  the reversible formation of oxaloacetate and adenosine triphosphate from  PEP, adenosine diphosphate and carbon dioxide, and uses Mn(2+) as the  activating metal ion.	transcription
55593	5	334985	6	NULL	NULL	0	NULL	statement 1			occurs simultaneously with					statement 2					NULL		0	NULL	NULL	NULL	abs-batch0740-0759_biochimie_88_6_16469427_s_2	16469427	Saccharomyces cerevisiae phosphoenolpyruvate (PEP) carboxykinase catalyzes  the reversible formation of oxaloacetate and adenosine triphosphate from  PEP, adenosine diphosphate and carbon dioxide, and uses Mn(2+) as the  activating metal ion.	transcription
52706	1	334987	5	NULL	NULL	0	NULL	PC	NULL		interacts with	NULL				cholesterol	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_chem-phys-lipids_22_3_719817_s_3	719817	The interactions of these  PC with cholesterol or desmosterol were studied.	transcription
52707	2	334987	5	NULL	NULL	0	NULL	PC	NULL		interacts with	NULL				desmosterol	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_chem-phys-lipids_22_3_719817_s_3	719817	The interactions of these  PC with cholesterol or desmosterol were studied.	transcription
55594	1	334987	6	NULL	NULL	0	NULL	PC			interacts with					cholesterol					NULL		0	NULL	NULL	NULL	abs-batch0650-0679_chem-phys-lipids_22_3_719817_s_3	719817	The interactions of these  PC with cholesterol or desmosterol were studied.	transcription
55595	2	334987	6	NULL	NULL	0	NULL	PC			interacts with					desmosterol					NULL		0	NULL	NULL	NULL	abs-batch0650-0679_chem-phys-lipids_22_3_719817_s_3	719817	The interactions of these  PC with cholesterol or desmosterol were studied.	transcription
52708	1	334988	5	NULL	NULL	0	NULL	IR	NULL	ligand-bound	associate with	NULL	selectively			DRMs	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_348_s_239	16249181	This may be related to the weaker membrane-ordering properties of desmosterol as suggested by the selective association of the ligand-bound IR with DRMs in the presence of cholesterol.	transcription
52709	2	334988	5	NULL	NULL	0	NULL	statement 1	NULL		in the presence of	NULL				cholesterol	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_348_s_239	16249181	This may be related to the weaker membrane-ordering properties of desmosterol as suggested by the selective association of the ligand-bound IR with DRMs in the presence of cholesterol.	transcription
55596	1	334988	6	NULL	NULL	0	NULL	IR		ligand bound	interacts with					DRMs					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_348_s_239	16249181	This may be related to the weaker membrane-ordering properties of desmosterol as suggested by the selective association of the ligand-bound IR with DRMs in the presence of cholesterol.	transcription
55597	2	334988	6	NULL	NULL	0	NULL	statement 1			occurs in the presence of					cholesterol					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_348_s_239	16249181	This may be related to the weaker membrane-ordering properties of desmosterol as suggested by the selective association of the ligand-bound IR with DRMs in the presence of cholesterol.	transcription
52710	1	334989	5	NULL	NULL	0	NULL	IR	NULL	ligand-occupied	associate with	NULL				DRMs	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_348_s_234	16249181	To study whether desmosterol interfered with the association of the ligand-occupied IR with DRMs, we stimulated cholesterol- or desmosterol-repleted HuH7 with insulin, lysed the cells in cold Triton X-100, and fractionated the material in an Optiprep gradient as described previously ( ).	transcription
52711	2	334989	5	NULL	NULL	0	NULL	desmosterol	NULL		interfere with	NULL	possibly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_348_s_234	16249181	To study whether desmosterol interfered with the association of the ligand-occupied IR with DRMs, we stimulated cholesterol- or desmosterol-repleted HuH7 with insulin, lysed the cells in cold Triton X-100, and fractionated the material in an Optiprep gradient as described previously ( ).	transcription
52712	1	334990	5	NULL	NULL	0	NULL	LXR	NULL		activates	NULL				stigmasterol	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_38_27816_s_264	16857673	We found that unsaturation of the cholesterol side chain was necessary and sufficient for the LXR-activating effects of stigmasterol: the presence of a double bond at C-20, C-22, and C-24 of cholesterol was associated with activation of LXR, with the delta24 bond in desmosterol having the most potent effect ( Fig. 2 B).	transcription
52713	2	334990	5	NULL	NULL	0	NULL	cholesterol	NULL	unsaturation of;;side chain of	is necessary for	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_38_27816_s_264	16857673	We found that unsaturation of the cholesterol side chain was necessary and sufficient for the LXR-activating effects of stigmasterol: the presence of a double bond at C-20, C-22, and C-24 of cholesterol was associated with activation of LXR, with the delta24 bond in desmosterol having the most potent effect ( Fig. 2 B).	transcription
52714	3	334990	5	NULL	NULL	0	NULL	cholesterol	NULL	unsaturation of;;side chain of	is sufficient for	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_38_27816_s_264	16857673	We found that unsaturation of the cholesterol side chain was necessary and sufficient for the LXR-activating effects of stigmasterol: the presence of a double bond at C-20, C-22, and C-24 of cholesterol was associated with activation of LXR, with the delta24 bond in desmosterol having the most potent effect ( Fig. 2 B).	transcription
55598	1	334990	6	NULL	NULL	0	NULL	LXR			activates					stigmasterol					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_38_27816_s_264	16857673	We found that unsaturation of the cholesterol side chain was necessary and sufficient for the LXR-activating effects of stigmasterol: the presence of a double bond at C-20, C-22, and C-24 of cholesterol was associated with activation of LXR, with the delta24 bond in desmosterol having the most potent effect ( Fig. 2 B).	transcription
55599	2	334990	6	NULL	NULL	0	NULL	cholesterol		unsaturation of	is necessary for			side chain		statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_38_27816_s_264	16857673	We found that unsaturation of the cholesterol side chain was necessary and sufficient for the LXR-activating effects of stigmasterol: the presence of a double bond at C-20, C-22, and C-24 of cholesterol was associated with activation of LXR, with the delta24 bond in desmosterol having the most potent effect ( Fig. 2 B).	transcription
52715	1	334992	5	NULL	NULL	0	NULL	taurine	NULL		inhibit	NULL				GlyRs	NULL	glycine current of	E53K;;D57K		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_50_50151_s_136	14525990	Co-application of taurine in the presence of 5 mM glycine demonstrated that taurine inhibited the glycine current of the E53K and D57K GlyRs.	transcription
52716	2	334992	5	NULL	NULL	0	NULL	statement 1	NULL		in the presence of	NULL				glycine	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_50_50151_s_136	14525990	Co-application of taurine in the presence of 5 mM glycine demonstrated that taurine inhibited the glycine current of the E53K and D57K GlyRs.	transcription
55600	1	334992	6	NULL	NULL	0	NULL	GlyR			exhibits			E53K		glycine current					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_50_50151_s_136	14525990	Co-application of taurine in the presence of 5 mM glycine demonstrated that taurine inhibited the glycine current of the E53K and D57K GlyRs.	transcription
55601	2	334992	6	NULL	NULL	0	NULL	GlyR			exhibits			D57K		glycine current					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_50_50151_s_136	14525990	Co-application of taurine in the presence of 5 mM glycine demonstrated that taurine inhibited the glycine current of the E53K and D57K GlyRs.	transcription
55602	3	334992	6	NULL	NULL	0	NULL	taurine			inhibits					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_50_50151_s_136	14525990	Co-application of taurine in the presence of 5 mM glycine demonstrated that taurine inhibited the glycine current of the E53K and D57K GlyRs.	transcription
55603	4	334992	6	NULL	NULL	0	NULL	taurine			inhibits					statement 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_50_50151_s_136	14525990	Co-application of taurine in the presence of 5 mM glycine demonstrated that taurine inhibited the glycine current of the E53K and D57K GlyRs.	transcription
52717	1	334993	5	NULL	NULL	0	NULL	glycine	NULL		activates	NULL				current	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_136_4_629_s_136	12055142	Figure 5 illustrates that although ethanol significantly inhibited the glycine-activated current, decanol had virtually no effect on the glycine current.	transcription
52718	2	334993	5	NULL	NULL	0	NULL	ethanol	NULL		inhibit	NULL	significantly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_136_4_629_s_136	12055142	Figure 5 illustrates that although ethanol significantly inhibited the glycine-activated current, decanol had virtually no effect on the glycine current.	transcription
52719	3	334993	5	NULL	NULL	0	NULL	decanol	NULL		does not effect	NULL				glycine current	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_136_4_629_s_136	12055142	Figure 5 illustrates that although ethanol significantly inhibited the glycine-activated current, decanol had virtually no effect on the glycine current.	transcription
55604	1	334993	6	NULL	NULL	0	NULL	ethanol			inhibits					glycine-activated current					NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_136_4_629_s_136	12055142	Figure 5 illustrates that although ethanol significantly inhibited the glycine-activated current, decanol had virtually no effect on the glycine current.	transcription
55605	2	334993	6	NULL	NULL	0	NULL	decanol			has no effect on					glycine-activated current					NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_136_4_629_s_136	12055142	Figure 5 illustrates that although ethanol significantly inhibited the glycine-activated current, decanol had virtually no effect on the glycine current.	transcription
52720	1	334994	5	NULL	NULL	0	NULL	glycine	NULL		is a component within	NULL				GpA	NULL		dimerization motif		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_49_50864_s_235	15448134	Substitution of these glycines (an important component within the dimerization motif in GpA) with alanines did not affect dimerization of N1 in the TOX-CAT assay ( Fig. 5 B and not shown).	transcription
52721	2	334994	5	NULL	NULL	0	NULL	statement 1	NULL		is substituted with	NULL				alanine	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_49_50864_s_235	15448134	Substitution of these glycines (an important component within the dimerization motif in GpA) with alanines did not affect dimerization of N1 in the TOX-CAT assay ( Fig. 5 B and not shown).	transcription
52722	3	334994	5	NULL	NULL	0	NULL	statement 2	NULL		does not affect	NULL				N1	NULL	dimerization of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_49_50864_s_235	15448134	Substitution of these glycines (an important component within the dimerization motif in GpA) with alanines did not affect dimerization of N1 in the TOX-CAT assay ( Fig. 5 B and not shown).	transcription
52723	1	334996	5	NULL	NULL	0	NULL	glycine	NULL		induce	NULL				ADE1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_7072_s_160	14645232	Glycine induction of  ADE1 and  SHM2 was confirmed by Northern analysis ( Fig. 5).	transcription
52724	2	334996	5	NULL	NULL	0	NULL	glycine	NULL		induce	NULL				SHM2	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_7072_s_160	14645232	Glycine induction of  ADE1 and  SHM2 was confirmed by Northern analysis ( Fig. 5).	transcription
55606	1	334996	6	NULL	NULL	0	NULL	glycine			induces					ADE1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_7072_s_160	14645232	Glycine induction of  ADE1 and  SHM2 was confirmed by Northern analysis ( Fig. 5).	transcription
55607	2	334996	6	NULL	NULL	0	NULL	glycine			induces					SHM2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_7072_s_160	14645232	Glycine induction of  ADE1 and  SHM2 was confirmed by Northern analysis ( Fig. 5).	transcription
52725	1	334997	5	NULL	NULL	0	NULL	Wy-14,643	NULL		induce	NULL				cells	NULL	proliferation of			NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_119	9934846	Since dietary glycine has been shown to inhibit Wy-14,643-induced cell proliferation and TNFalpha production ( 5), Kupffer cells were incubated with glycine prior to stimulation with Wy-14,643 to test the hypothesis that glycine inhibits superoxide production.	transcription
52726	2	334997	5	NULL	NULL	0	NULL	Wy-14,643	NULL		induce	NULL				TNFalpha	NULL	production of			NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_119	9934846	Since dietary glycine has been shown to inhibit Wy-14,643-induced cell proliferation and TNFalpha production ( 5), Kupffer cells were incubated with glycine prior to stimulation with Wy-14,643 to test the hypothesis that glycine inhibits superoxide production.	transcription
52727	3	334997	5	NULL	NULL	0	NULL	glycine	NULL	dietary	inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_119	9934846	Since dietary glycine has been shown to inhibit Wy-14,643-induced cell proliferation and TNFalpha production ( 5), Kupffer cells were incubated with glycine prior to stimulation with Wy-14,643 to test the hypothesis that glycine inhibits superoxide production.	transcription
52728	4	334997	5	NULL	NULL	0	NULL	glycine	NULL	dietary	inhibit	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_119	9934846	Since dietary glycine has been shown to inhibit Wy-14,643-induced cell proliferation and TNFalpha production ( 5), Kupffer cells were incubated with glycine prior to stimulation with Wy-14,643 to test the hypothesis that glycine inhibits superoxide production.	transcription
52729	5	334997	5	NULL	NULL	0	NULL	glycine	NULL		inhibit	NULL	possibly			superoxide	NULL	production of			NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_119	9934846	Since dietary glycine has been shown to inhibit Wy-14,643-induced cell proliferation and TNFalpha production ( 5), Kupffer cells were incubated with glycine prior to stimulation with Wy-14,643 to test the hypothesis that glycine inhibits superoxide production.	transcription
55608	1	334997	6	NULL	NULL	0	NULL	Wy-14,643			induces					cell proliferation					NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_119	9934846	Since dietary glycine has been shown to inhibit Wy-14,643-induced cell proliferation and TNFalpha production ( 5), Kupffer cells were incubated with glycine prior to stimulation with Wy-14,643 to test the hypothesis that glycine inhibits superoxide production.	transcription
55609	2	334997	6	NULL	NULL	0	NULL	dietary glycine			inhibits					statement 1					NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_119	9934846	Since dietary glycine has been shown to inhibit Wy-14,643-induced cell proliferation and TNFalpha production ( 5), Kupffer cells were incubated with glycine prior to stimulation with Wy-14,643 to test the hypothesis that glycine inhibits superoxide production.	transcription
55610	3	334997	6	NULL	NULL	0	NULL	Wy-14,643			induces					TNFalpha		production of 			NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_119	9934846	Since dietary glycine has been shown to inhibit Wy-14,643-induced cell proliferation and TNFalpha production ( 5), Kupffer cells were incubated with glycine prior to stimulation with Wy-14,643 to test the hypothesis that glycine inhibits superoxide production.	transcription
55611	4	334997	6	NULL	NULL	0	NULL	dietary glycine			inhibits					statement 2					NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_119	9934846	Since dietary glycine has been shown to inhibit Wy-14,643-induced cell proliferation and TNFalpha production ( 5), Kupffer cells were incubated with glycine prior to stimulation with Wy-14,643 to test the hypothesis that glycine inhibits superoxide production.	transcription
52730	1	334999	5	NULL	NULL	0	NULL	zmgrp5	NULL		is	NULL				Zea mays glycine-rich protein 5	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_plant-cell-rep_25_8_16528565_s_3	16528565	zmgrp5 (Zea mays glycine-rich protein  5) encodes a 187 amino acid glycine-rich protein that displays developmentally  regulated silk-specific expression.	transcription
52731	2	334999	5	NULL	NULL	0	NULL	zmgrp5	NULL		encodes	NULL				187 amino acid glycine-rich protein	NULL				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_plant-cell-rep_25_8_16528565_s_3	16528565	zmgrp5 (Zea mays glycine-rich protein  5) encodes a 187 amino acid glycine-rich protein that displays developmentally  regulated silk-specific expression.	transcription
52732	3	334999	5	NULL	NULL	0	NULL	zmgrp5	NULL		displays	NULL				silk-specific expression	NULL	developmentally regulated			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_plant-cell-rep_25_8_16528565_s_3	16528565	zmgrp5 (Zea mays glycine-rich protein  5) encodes a 187 amino acid glycine-rich protein that displays developmentally  regulated silk-specific expression.	transcription
55612	1	334999	6	NULL	NULL	0	NULL	zmgrp5			is					Zea mays glycine-rich protein 5					NULL		0	NULL	NULL	NULL	abs-batch0720-0739_plant-cell-rep_25_8_16528565_s_3	16528565	zmgrp5 (Zea mays glycine-rich protein  5) encodes a 187 amino acid glycine-rich protein that displays developmentally  regulated silk-specific expression.	transcription
55613	2	334999	6	NULL	NULL	0	NULL	zmgrp5			displays					silk-specific expression		developmentally regulated			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_plant-cell-rep_25_8_16528565_s_3	16528565	zmgrp5 (Zea mays glycine-rich protein  5) encodes a 187 amino acid glycine-rich protein that displays developmentally  regulated silk-specific expression.	transcription
55614	3	334999	6	NULL	NULL	0	NULL	zmgrp5			encodes					187 amino acid glycine-rich protein					NULL		0	NULL	NULL	NULL	abs-batch0720-0739_plant-cell-rep_25_8_16528565_s_3	16528565	zmgrp5 (Zea mays glycine-rich protein  5) encodes a 187 amino acid glycine-rich protein that displays developmentally  regulated silk-specific expression.	transcription
52733	1	335000	5	NULL	NULL	0	NULL	glycine	NULL		has affinity for	NULL				NMDA receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_brainresmolbrainres_57_1_10_s_219	9630479	Moreover, our results support the model that the effect of glycine on desensitization is a result of the affinity of glycine for the NMDA receptor because the rank order of glycine's ability to inhibit desensitization matched the rank order of the affinity of glycine determined for each combination [ 12,  30] (cf.  Table 1,  Fig. 5).	transcription
52734	1	335002	5	NULL	NULL	0	NULL	CYT1	NULL		is a type of	NULL				respiratory gene	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_7072_s_137	14645232	The glycine induction of a representative respiratory gene  CYT1, encoding cytochrome  c1, was confirmed by separate Northern analysis ( Fig. 5).	transcription
52735	2	335002	5	NULL	NULL	0	NULL	glycine	NULL		induce	NULL				CYT1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_7072_s_137	14645232	The glycine induction of a representative respiratory gene  CYT1, encoding cytochrome  c1, was confirmed by separate Northern analysis ( Fig. 5).	transcription
52736	3	335002	5	NULL	NULL	0	NULL	CYT1	NULL		encodes	NULL				cytochrome c1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_7072_s_137	14645232	The glycine induction of a representative respiratory gene  CYT1, encoding cytochrome  c1, was confirmed by separate Northern analysis ( Fig. 5).	transcription
56035	1	335002	6	NULL	NULL	0	NULL	CYT1			encodes for					cytochrome c1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_7072_s_137	14645232	The glycine induction of a representative respiratory gene  CYT1, encoding cytochrome  c1, was confirmed by separate Northern analysis ( Fig. 5).	transcription
56036	2	335002	6	NULL	NULL	0	NULL	CYT1			is a type of					respiratory gene					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_7072_s_137	14645232	The glycine induction of a representative respiratory gene  CYT1, encoding cytochrome  c1, was confirmed by separate Northern analysis ( Fig. 5).	transcription
56037	3	335002	6	NULL	NULL	0	NULL	glycine			induces					CYT1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_7072_s_137	14645232	The glycine induction of a representative respiratory gene  CYT1, encoding cytochrome  c1, was confirmed by separate Northern analysis ( Fig. 5).	transcription
52737	1	335003	5	NULL	NULL	0	NULL	ODC	NULL		is involved in	NULL		Lys-69		pyridoxal 5''-phosphate	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_41_30896_s_149	16916800	To note that the residue Lys-69 that in ODC is involved in the binding of pyridoxal 5''-phosphate is conserved in human ODCp, but it is substituted by glycine in murine ODCp.	transcription
52738	2	335003	5	NULL	NULL	0	NULL	statement 1	NULL		is conserved in	NULL				ODCp	NULL	human			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_41_30896_s_149	16916800	To note that the residue Lys-69 that in ODC is involved in the binding of pyridoxal 5''-phosphate is conserved in human ODCp, but it is substituted by glycine in murine ODCp.	transcription
52739	3	335003	5	NULL	NULL	0	NULL	statement 1	NULL		is substituted by	NULL				ODCp	NULL	murine	glycine		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_41_30896_s_149	16916800	To note that the residue Lys-69 that in ODC is involved in the binding of pyridoxal 5''-phosphate is conserved in human ODCp, but it is substituted by glycine in murine ODCp.	transcription
56038	1	335003	6	NULL	NULL	0	NULL	ODC			is involved in			Lys-69		pyridoxal 5''-phosphate		binding of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_41_30896_s_149	16916800	To note that the residue Lys-69 that in ODC is involved in the binding of pyridoxal 5''-phosphate is conserved in human ODCp, but it is substituted by glycine in murine ODCp.	transcription
52740	1	335004	5	NULL	NULL	0	NULL	GABAA blockers	NULL		induce	NULL				TH-P	NULL	strong			NULL		0	NULL	NULL	NULL	gw70_jneurosci_24_17_4242_s_164	15115820	In the absence of TTX, the GABAA and glycine blockers induced strong TH-P ( Fig. 5 b,f,j).	transcription
52741	2	335004	5	NULL	NULL	0	NULL	glycine blockers	NULL		induce	NULL				TH-P	NULL	strong			NULL		0	NULL	NULL	NULL	gw70_jneurosci_24_17_4242_s_164	15115820	In the absence of TTX, the GABAA and glycine blockers induced strong TH-P ( Fig. 5 b,f,j).	transcription
52742	3	335004	5	NULL	NULL	0	NULL	statement 1	NULL		in the absence of	NULL				TTX	NULL				NULL		0	NULL	NULL	NULL	gw70_jneurosci_24_17_4242_s_164	15115820	In the absence of TTX, the GABAA and glycine blockers induced strong TH-P ( Fig. 5 b,f,j).	transcription
52743	4	335004	5	NULL	NULL	0	NULL	statement 2	NULL		in the absence of	NULL				TTX	NULL				NULL		0	NULL	NULL	NULL	gw70_jneurosci_24_17_4242_s_164	15115820	In the absence of TTX, the GABAA and glycine blockers induced strong TH-P ( Fig. 5 b,f,j).	transcription
56039	1	335004	6	NULL	NULL	0	NULL	GABAA blockers			induce					TH-P		strong			NULL		0	NULL	NULL	NULL	gw70_jneurosci_24_17_4242_s_164	15115820	In the absence of TTX, the GABAA and glycine blockers induced strong TH-P ( Fig. 5 b,f,j).	transcription
56040	2	335004	6	NULL	NULL	0	NULL	glycine blockers			induce					TH-P		strong			NULL		0	NULL	NULL	NULL	gw70_jneurosci_24_17_4242_s_164	15115820	In the absence of TTX, the GABAA and glycine blockers induced strong TH-P ( Fig. 5 b,f,j).	transcription
56041	3	335004	6	NULL	NULL	0	NULL	statement 1			occurs in absence of					TTX					NULL		0	NULL	NULL	NULL	gw70_jneurosci_24_17_4242_s_164	15115820	In the absence of TTX, the GABAA and glycine blockers induced strong TH-P ( Fig. 5 b,f,j).	transcription
52744	1	335005	5	NULL	NULL	0	NULL	E. coli GJ146 derivatives	NULL		contain	NULL				pAT1	NULL				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_162_2_241_s_96	9627959	Similarly,  E. coli GJ146 derivatives containing pAT1 and pAT7 also showed osmoprotective effect of glycine betaine ( Fig. 5).	transcription
52745	2	335005	5	NULL	NULL	0	NULL	E. coli GJ146 derivatives	NULL		contain	NULL				pAT7	NULL				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_162_2_241_s_96	9627959	Similarly,  E. coli GJ146 derivatives containing pAT1 and pAT7 also showed osmoprotective effect of glycine betaine ( Fig. 5).	transcription
52746	3	335005	5	NULL	NULL	0	NULL	statement 1	NULL		displays	NULL				glycine betaine	NULL	osmoprotective effect of			NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_162_2_241_s_96	9627959	Similarly,  E. coli GJ146 derivatives containing pAT1 and pAT7 also showed osmoprotective effect of glycine betaine ( Fig. 5).	transcription
52747	4	335005	5	NULL	NULL	0	NULL	statement 2	NULL		displays	NULL				glycine betaine	NULL	osmoprotective effect of			NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_162_2_241_s_96	9627959	Similarly,  E. coli GJ146 derivatives containing pAT1 and pAT7 also showed osmoprotective effect of glycine betaine ( Fig. 5).	transcription
56042	1	335005	6	NULL	NULL	0	NULL	glycine betaine			shows					osmoprotective effects					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_162_2_241_s_96	9627959	Similarly,  E. coli GJ146 derivatives containing pAT1 and pAT7 also showed osmoprotective effect of glycine betaine ( Fig. 5).	transcription
56043	2	335005	6	NULL	NULL	0	NULL	pAT1			is a type of					E.coli GJ146 derivative					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_162_2_241_s_96	9627959	Similarly,  E. coli GJ146 derivatives containing pAT1 and pAT7 also showed osmoprotective effect of glycine betaine ( Fig. 5).	transcription
56044	3	335005	6	NULL	NULL	0	NULL	pAT7			is a type of					E.coli GJ146 derivative					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_162_2_241_s_96	9627959	Similarly,  E. coli GJ146 derivatives containing pAT1 and pAT7 also showed osmoprotective effect of glycine betaine ( Fig. 5).	transcription
56045	4	335005	6	NULL	NULL	0	NULL	pAT1			shows					statement 1					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_162_2_241_s_96	9627959	Similarly,  E. coli GJ146 derivatives containing pAT1 and pAT7 also showed osmoprotective effect of glycine betaine ( Fig. 5).	transcription
56046	5	335005	6	NULL	NULL	0	NULL	pAT7			shows					statement 1					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_162_2_241_s_96	9627959	Similarly,  E. coli GJ146 derivatives containing pAT1 and pAT7 also showed osmoprotective effect of glycine betaine ( Fig. 5).	transcription
52748	1	335006	5	NULL	NULL	0	NULL	taurine	NULL	release of	is induced by	NULL				hyposmosis	NULL				NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_1_s_104	10536255	The hyposmotically induced releases of taurine, glutamate, glycine or phosphoethanolamine were not affected by PMA ( Fig. 4,  Fig. 5 and  Fig. 6).	transcription
52749	2	335006	5	NULL	NULL	0	NULL	glutamate	NULL	release of	is induced by	NULL				hyposmosis	NULL				NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_1_s_104	10536255	The hyposmotically induced releases of taurine, glutamate, glycine or phosphoethanolamine were not affected by PMA ( Fig. 4,  Fig. 5 and  Fig. 6).	transcription
52750	3	335006	5	NULL	NULL	0	NULL	glycine	NULL	release of	is induced by	NULL				hyposmosis	NULL				NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_1_s_104	10536255	The hyposmotically induced releases of taurine, glutamate, glycine or phosphoethanolamine were not affected by PMA ( Fig. 4,  Fig. 5 and  Fig. 6).	transcription
52751	4	335006	5	NULL	NULL	0	NULL	phosphoethanolamine	NULL	release of	is induced by	NULL				hyposmosis	NULL				NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_1_s_104	10536255	The hyposmotically induced releases of taurine, glutamate, glycine or phosphoethanolamine were not affected by PMA ( Fig. 4,  Fig. 5 and  Fig. 6).	transcription
52752	5	335006	5	NULL	NULL	0	NULL	PMA	NULL		does not affect	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_1_s_104	10536255	The hyposmotically induced releases of taurine, glutamate, glycine or phosphoethanolamine were not affected by PMA ( Fig. 4,  Fig. 5 and  Fig. 6).	transcription
52753	6	335006	5	NULL	NULL	0	NULL	PMA	NULL		does not affect	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_1_s_104	10536255	The hyposmotically induced releases of taurine, glutamate, glycine or phosphoethanolamine were not affected by PMA ( Fig. 4,  Fig. 5 and  Fig. 6).	transcription
52754	7	335006	5	NULL	NULL	0	NULL	PMA	NULL		does not affect	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_1_s_104	10536255	The hyposmotically induced releases of taurine, glutamate, glycine or phosphoethanolamine were not affected by PMA ( Fig. 4,  Fig. 5 and  Fig. 6).	transcription
52755	8	335006	5	NULL	NULL	0	NULL	PMA	NULL		does not affect	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_1_s_104	10536255	The hyposmotically induced releases of taurine, glutamate, glycine or phosphoethanolamine were not affected by PMA ( Fig. 4,  Fig. 5 and  Fig. 6).	transcription
56047	1	335006	6	NULL	NULL	0	NULL	hyposomosis			induces					taurine		release of			NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_1_s_104	10536255	The hyposmotically induced releases of taurine, glutamate, glycine or phosphoethanolamine were not affected by PMA ( Fig. 4,  Fig. 5 and  Fig. 6).	transcription
56048	2	335006	6	NULL	NULL	0	NULL	hyposomosis			induces					glutamate		release of			NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_1_s_104	10536255	The hyposmotically induced releases of taurine, glutamate, glycine or phosphoethanolamine were not affected by PMA ( Fig. 4,  Fig. 5 and  Fig. 6).	transcription
56049	3	335006	6	NULL	NULL	0	NULL	hyposomosis			induces					glycine		release of			NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_1_s_104	10536255	The hyposmotically induced releases of taurine, glutamate, glycine or phosphoethanolamine were not affected by PMA ( Fig. 4,  Fig. 5 and  Fig. 6).	transcription
56050	4	335006	6	NULL	NULL	0	NULL	hyposomosis			induces					phosphoethanolamine		release of			NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_1_s_104	10536255	The hyposmotically induced releases of taurine, glutamate, glycine or phosphoethanolamine were not affected by PMA ( Fig. 4,  Fig. 5 and  Fig. 6).	transcription
56051	5	335006	6	NULL	NULL	0	NULL	statement 1			is not affected by					PMA					NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_1_s_104	10536255	The hyposmotically induced releases of taurine, glutamate, glycine or phosphoethanolamine were not affected by PMA ( Fig. 4,  Fig. 5 and  Fig. 6).	transcription
56052	6	335006	6	NULL	NULL	0	NULL	statement 2			is not affected by					PMA					NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_1_s_104	10536255	The hyposmotically induced releases of taurine, glutamate, glycine or phosphoethanolamine were not affected by PMA ( Fig. 4,  Fig. 5 and  Fig. 6).	transcription
56053	7	335006	6	NULL	NULL	0	NULL	statement 3			is not affected by					PMA					NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_1_s_104	10536255	The hyposmotically induced releases of taurine, glutamate, glycine or phosphoethanolamine were not affected by PMA ( Fig. 4,  Fig. 5 and  Fig. 6).	transcription
56054	8	335006	6	NULL	NULL	0	NULL	statement 4			is not affected by					PMA					NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_1_s_104	10536255	The hyposmotically induced releases of taurine, glutamate, glycine or phosphoethanolamine were not affected by PMA ( Fig. 4,  Fig. 5 and  Fig. 6).	transcription
52756	1	335007	5	NULL	NULL	0	NULL	glycine	NULL		is added to	NULL				WY-14,643 diet	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_11_2075_s_97	10545408	The addition of 5% glycine to the WY-14,643 diet did not affect the development of preneoplastic foci in either of these groups.	transcription
52757	2	335007	5	NULL	NULL	0	NULL	statement 1	NULL		does not affect	NULL				preneoplastic foci	NULL	development of			NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_11_2075_s_97	10545408	The addition of 5% glycine to the WY-14,643 diet did not affect the development of preneoplastic foci in either of these groups.	transcription
52758	1	335008	5	NULL	NULL	0	NULL	glycine	NULL		inhibit	NULL				tumors	NULL	growth of;;large			NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_11_2075_s_181	10545408	In these studies, glycine inhibited the growth of larger tumors to a greater extent than smaller tumors (Figure 5  ).	transcription
52759	2	335008	5	NULL	NULL	0	NULL	glycine	NULL		inhibit	NULL				tumors	NULL	growth of;;small			NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_11_2075_s_181	10545408	In these studies, glycine inhibited the growth of larger tumors to a greater extent than smaller tumors (Figure 5  ).	transcription
52760	3	335008	5	NULL	NULL	0	NULL	statement 1	NULL		greater extent than	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_11_2075_s_181	10545408	In these studies, glycine inhibited the growth of larger tumors to a greater extent than smaller tumors (Figure 5  ).	transcription
56055	1	335008	6	NULL	NULL	0	NULL	glycine			inhibits					tumors		growth of;; larger			NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_11_2075_s_181	10545408	In these studies, glycine inhibited the growth of larger tumors to a greater extent than smaller tumors (Figure 5  ).	transcription
56056	2	335008	6	NULL	NULL	0	NULL	glycine			inhibits					tumors		growth of;; smaller			NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_11_2075_s_181	10545408	In these studies, glycine inhibited the growth of larger tumors to a greater extent than smaller tumors (Figure 5  ).	transcription
56057	3	335008	6	NULL	NULL	0	NULL	statement 1			is greater than					statement 2					NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_11_2075_s_181	10545408	In these studies, glycine inhibited the growth of larger tumors to a greater extent than smaller tumors (Figure 5  ).	transcription
52761	1	335009	5	NULL	NULL	0	NULL	Kupffer cells	NULL		produce	NULL				superoxide	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_120	9934846	Indeed, glycine prevented Wy-14,643-stimulated superoxide production by Kupffer cells (Figure 5  ).	transcription
52762	2	335009	5	NULL	NULL	0	NULL	Wy-14,643	NULL		stimulates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_120	9934846	Indeed, glycine prevented Wy-14,643-stimulated superoxide production by Kupffer cells (Figure 5  ).	transcription
52763	3	335009	5	NULL	NULL	0	NULL	glycine	NULL		prevents	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_120	9934846	Indeed, glycine prevented Wy-14,643-stimulated superoxide production by Kupffer cells (Figure 5  ).	transcription
56058	1	335009	6	NULL	NULL	0	NULL	Wy-14,643			stimulates					superoxide		production of			NULL	Kupffer cells	0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_120	9934846	Indeed, glycine prevented Wy-14,643-stimulated superoxide production by Kupffer cells (Figure 5  ).	transcription
56059	2	335009	6	NULL	NULL	0	NULL	glycine			prevents					statement 1					NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_120	9934846	Indeed, glycine prevented Wy-14,643-stimulated superoxide production by Kupffer cells (Figure 5  ).	transcription
52764	1	335010	5	NULL	NULL	0	NULL	proline porter II	NULL		is a type of	NULL				transporter	NULL				NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_230_s_2110	10066837	Insertion  proQ220::Tn 5 alters regulation of proline porter II, a transporter of proline and glycine betaine in  Escherichia coli.	transcription
52765	2	335010	5	NULL	NULL	0	NULL	proline porter II	NULL		transports	NULL				proline	NULL				NULL	Escherichia coli	0	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_230_s_2110	10066837	Insertion  proQ220::Tn 5 alters regulation of proline porter II, a transporter of proline and glycine betaine in  Escherichia coli.	transcription
52766	3	335010	5	NULL	NULL	0	NULL	proline porter II	NULL		transports	NULL				glycine betaine	NULL				NULL	Escherichia coli	0	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_230_s_2110	10066837	Insertion  proQ220::Tn 5 alters regulation of proline porter II, a transporter of proline and glycine betaine in  Escherichia coli.	transcription
52767	4	335010	5	NULL	NULL	0	NULL	proQ220::Tn 5	NULL	insertion of	alters	NULL				proline porter II	NULL	regulation of			NULL	Escherichia coli	NULL	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_230_s_2110	10066837	Insertion  proQ220::Tn 5 alters regulation of proline porter II, a transporter of proline and glycine betaine in  Escherichia coli.	transcription
56062	1	335010	6	NULL	NULL	0	NULL	proline porter II			is a type of					proline transporter					NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_230_s_2110	10066837	Insertion  proQ220::Tn 5 alters regulation of proline porter II, a transporter of proline and glycine betaine in  Escherichia coli.	transcription
56063	2	335010	6	NULL	NULL	0	NULL	proline porter II			is a type of					glycine betaine transporter					NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_230_s_2110	10066837	Insertion  proQ220::Tn 5 alters regulation of proline porter II, a transporter of proline and glycine betaine in  Escherichia coli.	transcription
56064	3	335010	6	NULL	NULL	0	NULL	proQ220::Tn 5		insertion of 	alters 					proline porter II		regulation of 			NULL		0	NULL	NULL	NULL	gw60_microbiolmolbiolr_63_1_230_s_2110	10066837	Insertion  proQ220::Tn 5 alters regulation of proline porter II, a transporter of proline and glycine betaine in  Escherichia coli.	transcription
52768	1	335011	5	NULL	NULL	0	NULL	E7	NULL		stimulates	NULL				VAI	NULL	expression of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_7_4927_s_194	10373542	Indeed, substitution of the C24 residue to glycine is sufficient to abrogate the ability of E7 to stimulate VAI expression (lane 5).	transcription
52769	2	335011	5	NULL	NULL	0	NULL		NULL		is substituted to	NULL		C24 residue			NULL		glycine		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_7_4927_s_194	10373542	Indeed, substitution of the C24 residue to glycine is sufficient to abrogate the ability of E7 to stimulate VAI expression (lane 5).	transcription
52770	3	335011	5	NULL	NULL	0	NULL	statement 2	NULL		abrogates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_7_4927_s_194	10373542	Indeed, substitution of the C24 residue to glycine is sufficient to abrogate the ability of E7 to stimulate VAI expression (lane 5).	transcription
56065	1	335011	6	NULL	NULL	0	NULL	E7			stimulate					VAI		expression of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_7_4927_s_194	10373542	Indeed, substitution of the C24 residue to glycine is sufficient to abrogate the ability of E7 to stimulate VAI expression (lane 5).	transcription
56066	2	335011	6	NULL	NULL	0	NULL			substitution of 	abrogates			C24		statement 1					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_7_4927_s_194	10373542	Indeed, substitution of the C24 residue to glycine is sufficient to abrogate the ability of E7 to stimulate VAI expression (lane 5).	transcription
52771	1	335012	5	NULL	NULL	0	NULL	GFRs	NULL	decrease in	is caused by	NULL				CsA	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_56_3_455_s_97	10462532	This effect appears specific for glycine, because dietary valine (5%) did not block decreases in GFRs caused by CsA.	transcription
52772	2	335012	5	NULL	NULL	0	NULL	valine	NULL	dietary	does not block	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_56_3_455_s_97	10462532	This effect appears specific for glycine, because dietary valine (5%) did not block decreases in GFRs caused by CsA.	transcription
56067	1	335012	6	NULL	NULL	0	NULL	CsA			causes					GFR		decrease in			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_56_3_455_s_97	10462532	This effect appears specific for glycine, because dietary valine (5%) did not block decreases in GFRs caused by CsA.	transcription
56068	2	335012	6	NULL	NULL	0	NULL			dietary 	does not block			valine		statement 1					NULL		0	NULL	NULL	NULL	gw60_molpharmacol_56_3_455_s_97	10462532	This effect appears specific for glycine, because dietary valine (5%) did not block decreases in GFRs caused by CsA.	transcription
52773	1	335013	5	NULL	NULL	0	NULL	glycine	NULL	medium	effect	NULL	may			thymidylate	NULL	biosynthesis of			NULL	MCF-7 cells	0	NULL	NULL	NULL	gw60_jbiolchem_277_41_38381_s_194	12161434	The effect of medium glycine on thymidylate biosynthesis was determined for MCF-7 cells and MCF-7 cells that express GlyT (Fig.  5).	transcription
52774	2	335013	5	NULL	NULL	0	NULL	glycine	NULL	medium	effect	NULL	may			thymidylate	NULL	biosynthesis of			NULL	MCF-7 cells that express GlyT	0	NULL	NULL	NULL	gw60_jbiolchem_277_41_38381_s_194	12161434	The effect of medium glycine on thymidylate biosynthesis was determined for MCF-7 cells and MCF-7 cells that express GlyT (Fig.  5).	transcription
56069	1	335013	6	NULL	NULL	0	NULL	MCF-7 cells			express					GlyT					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_41_38381_s_194	12161434	The effect of medium glycine on thymidylate biosynthesis was determined for MCF-7 cells and MCF-7 cells that express GlyT (Fig.  5).	transcription
52775	1	335014	5	NULL	NULL	0	NULL	leucine	NULL	uptake of	is inhibited by	NULL				glycine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_28_19745_s_124	10391916	As shown in Fig.  5 a, the leucine uptake was inhibited by glycine and L-isomers of the neutral amino acids and histidine.	transcription
52776	2	335014	5	NULL	NULL	0	NULL	leucine	NULL	uptake of	is inhibited by	NULL				L-isomers of neutral amino acids	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_28_19745_s_124	10391916	As shown in Fig.  5 a, the leucine uptake was inhibited by glycine and L-isomers of the neutral amino acids and histidine.	transcription
52777	3	335014	5	NULL	NULL	0	NULL	leucine	NULL	uptake of	is inhibited by	NULL				histidine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_28_19745_s_124	10391916	As shown in Fig.  5 a, the leucine uptake was inhibited by glycine and L-isomers of the neutral amino acids and histidine.	transcription
56070	1	335014	6	NULL	NULL	0	NULL	glycine			inhibits					leucine		uptake of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_28_19745_s_124	10391916	As shown in Fig.  5 a, the leucine uptake was inhibited by glycine and L-isomers of the neutral amino acids and histidine.	transcription
56071	2	335014	6	NULL	NULL	0	NULL	histidine			inhibits					leucine		uptake of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_28_19745_s_124	10391916	As shown in Fig.  5 a, the leucine uptake was inhibited by glycine and L-isomers of the neutral amino acids and histidine.	transcription
52778	1	335015	5	NULL	NULL	0	NULL		NULL	MTSET modification of	increases	NULL	dramatically	R271C		glycine	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_8_2589_s_385	11306612	MTSET modification of R271C, A272C, S273C, L274C, and K276C dramatically increased the apparent glycine affinity (Fig.  5 B).	transcription
52779	2	335015	5	NULL	NULL	0	NULL		NULL	MTSET modification of	increases	NULL	dramatically	A272C		glycine	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_8_2589_s_385	11306612	MTSET modification of R271C, A272C, S273C, L274C, and K276C dramatically increased the apparent glycine affinity (Fig.  5 B).	transcription
52780	3	335015	5	NULL	NULL	0	NULL		NULL	MTSET modification of	increases	NULL	dramatically	S273C		glycine	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_8_2589_s_385	11306612	MTSET modification of R271C, A272C, S273C, L274C, and K276C dramatically increased the apparent glycine affinity (Fig.  5 B).	transcription
52781	4	335015	5	NULL	NULL	0	NULL		NULL	MTSET modification of	increases	NULL	dramatically	L274C		glycine	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_8_2589_s_385	11306612	MTSET modification of R271C, A272C, S273C, L274C, and K276C dramatically increased the apparent glycine affinity (Fig.  5 B).	transcription
52782	5	335015	5	NULL	NULL	0	NULL		NULL	MTSET modification of	increases	NULL	dramatically	K276C 		glycine	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_8_2589_s_385	11306612	MTSET modification of R271C, A272C, S273C, L274C, and K276C dramatically increased the apparent glycine affinity (Fig.  5 B).	transcription
56072	1	335015	6	NULL	NULL	0	NULL			modification of 	increases			R271C		glycine		affinity of 			NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_8_2589_s_385	11306612	MTSET modification of R271C, A272C, S273C, L274C, and K276C dramatically increased the apparent glycine affinity (Fig.  5 B).	transcription
56073	2	335015	6	NULL	NULL	0	NULL			modification of	increases			A272C		glycine		affinity of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_8_2589_s_385	11306612	MTSET modification of R271C, A272C, S273C, L274C, and K276C dramatically increased the apparent glycine affinity (Fig.  5 B).	transcription
56074	3	335015	6	NULL	NULL	0	NULL			modification of	increases			S273C		glycine		affinity of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_8_2589_s_385	11306612	MTSET modification of R271C, A272C, S273C, L274C, and K276C dramatically increased the apparent glycine affinity (Fig.  5 B).	transcription
56075	4	335015	6	NULL	NULL	0	NULL			modification of	increases			L274C		glycine		affinity of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_8_2589_s_385	11306612	MTSET modification of R271C, A272C, S273C, L274C, and K276C dramatically increased the apparent glycine affinity (Fig.  5 B).	transcription
56082	5	335015	6	NULL	NULL	0	NULL			modification of	increases			K276C		glycine		affinity of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_8_2589_s_385	11306612	MTSET modification of R271C, A272C, S273C, L274C, and K276C dramatically increased the apparent glycine affinity (Fig.  5 B).	transcription
52783	1	335016	5	NULL	NULL	0	NULL	L-threonine	NULL		is interconverted to	NULL				glycine	NULL				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_appl-microbiol-biotechnol_68_4_15726349_s_3	15726349	This aldolase is a pyridoxal 5''-phosphate-dependent enzyme  that stereospecifically catalyzes the interconversion of L-threonine to  glycine and acetaldehyde.	transcription
52784	2	335016	5	NULL	NULL	0	NULL	L-threonine	NULL		is interconverted to	NULL				acetaldehyde	NULL				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_appl-microbiol-biotechnol_68_4_15726349_s_3	15726349	This aldolase is a pyridoxal 5''-phosphate-dependent enzyme  that stereospecifically catalyzes the interconversion of L-threonine to  glycine and acetaldehyde.	transcription
56083	1	335016	6	NULL	NULL	0	NULL	L-threonine			is converted to					glycine					NULL		0	NULL	NULL	NULL	abs-batch0530-0539_appl-microbiol-biotechnol_68_4_15726349_s_3	15726349	This aldolase is a pyridoxal 5''-phosphate-dependent enzyme  that stereospecifically catalyzes the interconversion of L-threonine to  glycine and acetaldehyde.	transcription
56084	2	335016	6	NULL	NULL	0	NULL	L-threonine			is converted to					acetaldehyde					NULL		0	NULL	NULL	NULL	abs-batch0530-0539_appl-microbiol-biotechnol_68_4_15726349_s_3	15726349	This aldolase is a pyridoxal 5''-phosphate-dependent enzyme  that stereospecifically catalyzes the interconversion of L-threonine to  glycine and acetaldehyde.	transcription
56085	3	335016	6	NULL	NULL	0	NULL	pyridoxal 5''-phosphate-dependent enzyme			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	abs-batch0530-0539_appl-microbiol-biotechnol_68_4_15726349_s_3	15726349	This aldolase is a pyridoxal 5''-phosphate-dependent enzyme  that stereospecifically catalyzes the interconversion of L-threonine to  glycine and acetaldehyde.	transcription
56086	4	335016	6	NULL	NULL	0	NULL	pyridoxal 5''-phosphate-dependent enzyme			catalyzes					statement 2					NULL		0	NULL	NULL	NULL	abs-batch0530-0539_appl-microbiol-biotechnol_68_4_15726349_s_3	15726349	This aldolase is a pyridoxal 5''-phosphate-dependent enzyme  that stereospecifically catalyzes the interconversion of L-threonine to  glycine and acetaldehyde.	transcription
56087	5	335016	6	NULL	NULL	0	NULL	pyridoxal 5''-phosphate-dependent enzyme			is a type of					aldolase					NULL		0	NULL	NULL	NULL	abs-batch0530-0539_appl-microbiol-biotechnol_68_4_15726349_s_3	15726349	This aldolase is a pyridoxal 5''-phosphate-dependent enzyme  that stereospecifically catalyzes the interconversion of L-threonine to  glycine and acetaldehyde.	transcription
52785	1	335017	5	NULL	NULL	0	NULL	NMDA receptors	NULL	activation of	requires	NULL				glycine	NULL	presence of			NULL		0	NULL	NULL	NULL	gw70_brainres_1020_1_178_s_146	15312801	Finally, the activation of NMDA receptors often requires the presence of glycine  [  15], but bath application of glycine (20  M) in these experiments produced no significant  changes in mean sEPSC amplitude or shape ( n=5).	transcription
56088	1	335017	6	NULL	NULL	0	NULL	NMDA receptor		activation of 	requires					glycine		presence of 			NULL		0	NULL	NULL	NULL	gw70_brainres_1020_1_178_s_146	15312801	Finally, the activation of NMDA receptors often requires the presence of glycine  [  15], but bath application of glycine (20  M) in these experiments produced no significant  changes in mean sEPSC amplitude or shape ( n=5).	transcription
52786	1	335018	5	NULL	NULL	0	NULL	currents	NULL		is induced by	NULL				glycine	NULL				NULL		0	NULL	NULL	NULL	gw70_molpharmacol_69_3_991_s_149	16332990	As illustrated in  Fig. 6C, whereas the currents induced by 5 muM glycine were markedly enhanced by 300 nM THC, the  IGly level induced by 30 muM glycine remained unchanged in the presence of THC ( Fig. 6C).	transcription
52787	2	335018	5	NULL	NULL	0	NULL	THC	NULL		enhance	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_molpharmacol_69_3_991_s_149	16332990	As illustrated in  Fig. 6C, whereas the currents induced by 5 muM glycine were markedly enhanced by 300 nM THC, the  IGly level induced by 30 muM glycine remained unchanged in the presence of THC ( Fig. 6C).	transcription
52788	3	335018	5	NULL	NULL	0	NULL	IGly	NULL	levels of	is induced by	NULL				glycine	NULL				NULL		0	NULL	NULL	NULL	gw70_molpharmacol_69_3_991_s_149	16332990	As illustrated in  Fig. 6C, whereas the currents induced by 5 muM glycine were markedly enhanced by 300 nM THC, the  IGly level induced by 30 muM glycine remained unchanged in the presence of THC ( Fig. 6C).	transcription
52789	4	335018	5	NULL	NULL	0	NULL	THC	NULL		does not effect	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw70_molpharmacol_69_3_991_s_149	16332990	As illustrated in  Fig. 6C, whereas the currents induced by 5 muM glycine were markedly enhanced by 300 nM THC, the  IGly level induced by 30 muM glycine remained unchanged in the presence of THC ( Fig. 6C).	transcription
56089	1	335018	6	NULL	NULL	0	NULL	glycine			induces					currents					NULL		0	NULL	NULL	NULL	gw70_molpharmacol_69_3_991_s_149	16332990	As illustrated in  Fig. 6C, whereas the currents induced by 5 muM glycine were markedly enhanced by 300 nM THC, the  IGly level induced by 30 muM glycine remained unchanged in the presence of THC ( Fig. 6C).	transcription
56090	2	335018	6	NULL	NULL	0	NULL	THC			enhances					statement 1					NULL		0	NULL	NULL	NULL	gw70_molpharmacol_69_3_991_s_149	16332990	As illustrated in  Fig. 6C, whereas the currents induced by 5 muM glycine were markedly enhanced by 300 nM THC, the  IGly level induced by 30 muM glycine remained unchanged in the presence of THC ( Fig. 6C).	transcription
52790	1	335019	5	NULL	NULL	0	NULL	MTX	NULL		induce	NULL				K+ 	NULL	release of			NULL		0	NULL	NULL	NULL	gw70_molpharmacol_66_4_909_s_213	15385641	We also tested the ability of MTX to induce K+ release in the presence or absence of glycine and found that 5 mM extracellular glycine did not affect the MTX-induced cation fluxes ( Fig. 5E).	transcription
52791	2	335019	5	NULL	NULL	0	NULL	MTX	NULL		induce	NULL				cation fluxes	NULL				NULL		0	NULL	NULL	NULL	gw70_molpharmacol_66_4_909_s_213	15385641	We also tested the ability of MTX to induce K+ release in the presence or absence of glycine and found that 5 mM extracellular glycine did not affect the MTX-induced cation fluxes ( Fig. 5E).	transcription
52792	3	335019	5	NULL	NULL	0	NULL	glycine	NULL		does not affect	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_molpharmacol_66_4_909_s_213	15385641	We also tested the ability of MTX to induce K+ release in the presence or absence of glycine and found that 5 mM extracellular glycine did not affect the MTX-induced cation fluxes ( Fig. 5E).	transcription
56091	1	335019	6	NULL	NULL	0	NULL	MTX			induces					cation flux					NULL		0	NULL	NULL	NULL	gw70_molpharmacol_66_4_909_s_213	15385641	We also tested the ability of MTX to induce K+ release in the presence or absence of glycine and found that 5 mM extracellular glycine did not affect the MTX-induced cation fluxes ( Fig. 5E).	transcription
56092	2	335019	6	NULL	NULL	0	NULL	glycine		extracellular	does not affect					statement 1					NULL		0	NULL	NULL	NULL	gw70_molpharmacol_66_4_909_s_213	15385641	We also tested the ability of MTX to induce K+ release in the presence or absence of glycine and found that 5 mM extracellular glycine did not affect the MTX-induced cation fluxes ( Fig. 5E).	transcription
52793	1	335020	5	NULL	NULL	0	NULL	glycine	NULL		activates	NULL				glycine receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_9_5883_s_277	11500467	These data are consistent with the hypothesis that glycine activates a glycine receptor (Fig.  5), leading to the influx of chloride which hyperpolarizes the macrophage membrane and decreases the opening time of voltage-dependent calcium channels.	transcription
52794	2	335020	5	NULL	NULL	0	NULL	statement 1	NULL		leads to	NULL				chloride	NULL	influx of			NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_9_5883_s_277	11500467	These data are consistent with the hypothesis that glycine activates a glycine receptor (Fig.  5), leading to the influx of chloride which hyperpolarizes the macrophage membrane and decreases the opening time of voltage-dependent calcium channels.	transcription
52795	3	335020	5	NULL	NULL	0	NULL	chloride	NULL		hyperpolarizes	NULL				macrophage membrane	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_9_5883_s_277	11500467	These data are consistent with the hypothesis that glycine activates a glycine receptor (Fig.  5), leading to the influx of chloride which hyperpolarizes the macrophage membrane and decreases the opening time of voltage-dependent calcium channels.	transcription
52796	4	335020	5	NULL	NULL	0	NULL	chloride	NULL		decreases	NULL				calcium channels	NULL	opening time of			NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_9_5883_s_277	11500467	These data are consistent with the hypothesis that glycine activates a glycine receptor (Fig.  5), leading to the influx of chloride which hyperpolarizes the macrophage membrane and decreases the opening time of voltage-dependent calcium channels.	transcription
52797	5	335020	5	NULL	NULL	0	NULL	calcium channels	NULL		is dependent on	NULL				voltage	NULL				NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_9_5883_s_277	11500467	These data are consistent with the hypothesis that glycine activates a glycine receptor (Fig.  5), leading to the influx of chloride which hyperpolarizes the macrophage membrane and decreases the opening time of voltage-dependent calcium channels.	transcription
56093	1	335020	6	NULL	NULL	0	NULL	glycine			activates					glycine receptor					NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_9_5883_s_277	11500467	These data are consistent with the hypothesis that glycine activates a glycine receptor (Fig.  5), leading to the influx of chloride which hyperpolarizes the macrophage membrane and decreases the opening time of voltage-dependent calcium channels.	transcription
56094	2	335020	6	NULL	NULL	0	NULL	statement 1			leads to					chloride		influx of 			NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_9_5883_s_277	11500467	These data are consistent with the hypothesis that glycine activates a glycine receptor (Fig.  5), leading to the influx of chloride which hyperpolarizes the macrophage membrane and decreases the opening time of voltage-dependent calcium channels.	transcription
56095	3	335020	6	NULL	NULL	0	NULL	chloride		influx of	hyperpolarizes					macrophage membrane					NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_9_5883_s_277	11500467	These data are consistent with the hypothesis that glycine activates a glycine receptor (Fig.  5), leading to the influx of chloride which hyperpolarizes the macrophage membrane and decreases the opening time of voltage-dependent calcium channels.	transcription
56096	4	335020	6	NULL	NULL	0	NULL	chloride		influx of	decreases					calcium channels		opening time;; voltage dependent			NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_9_5883_s_277	11500467	These data are consistent with the hypothesis that glycine activates a glycine receptor (Fig.  5), leading to the influx of chloride which hyperpolarizes the macrophage membrane and decreases the opening time of voltage-dependent calcium channels.	transcription
52798	1	335021	5	NULL	NULL	0	NULL	DCS	NULL	increased efficacy of	is elicited through	NULL	solely				NULL		glycine binding site		NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_41_2_151_s_155	11489451	Interestingly,  Fig. 5 also indicates that the increased efficacy of DCS in comparison to glycine controls for NMDA receptors containing NR2C subunits is elicited solely through the glycine binding site.	transcription
53350	1	335023	7	NULL	NULL	0	NULL	receptor glycine	NULL	affinity of	is reduced in	NULL				acutely dissociated hippocampal neurons	NULL				NULL	mice carrying Grin1 D481N mutations	NULL	NULL	NULL	NULL	gw60_jneurosci_20_11_4037_s_3	10818139	Glycine concentration-response curves from acutely dissociated hippocampal neurons revealed a 5- and 86-fold reduction in receptor glycine affinity in mice carrying  Grin1 D481N and  Grin1K483Qmutations, respectively, whereas receptor glutamate affinity remained unaffected.	transcription
53351	2	335023	7	NULL	NULL	0	NULL	receptor glycine	NULL	affinity of	reduced in	NULL				acutely dissociated hippocampal neurons	NULL				NULL	 mice carrying Grin1K483Qmutations	0	NULL	NULL	NULL	gw60_jneurosci_20_11_4037_s_3	10818139	Glycine concentration-response curves from acutely dissociated hippocampal neurons revealed a 5- and 86-fold reduction in receptor glycine affinity in mice carrying  Grin1 D481N and  Grin1K483Qmutations, respectively, whereas receptor glutamate affinity remained unaffected.	transcription
53352	3	335023	7	NULL	NULL	0	NULL	receptor glutamate	NULL	affinity of	is not affected in	NULL				 acutely dissociated hippocampal neurons	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_11_4037_s_3	10818139	Glycine concentration-response curves from acutely dissociated hippocampal neurons revealed a 5- and 86-fold reduction in receptor glycine affinity in mice carrying  Grin1 D481N and  Grin1K483Qmutations, respectively, whereas receptor glutamate affinity remained unaffected.	transcription
53368	1	335024	5	NULL	NULL	0	NULL	ischemia	NULL		induce	NULL				glycine	NULL	release of			NULL	in vitro	0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_553_s_69	15020253	The present finding that in vitro ischemia induces glycine release with an extent  comparable to that of GABA release demonstrates that no involvement of glycine receptors  in inhibiting the release of  -glutamate following in vitro ischemia [ 5] is due to the absence of presynaptic glycine receptors leading to the inhibition.	transcription
53369	2	335024	5	NULL	NULL	0	NULL	ischemia	NULL		induce	NULL				GABA	NULL	release of			NULL	in vitro	0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_553_s_69	15020253	The present finding that in vitro ischemia induces glycine release with an extent  comparable to that of GABA release demonstrates that no involvement of glycine receptors  in inhibiting the release of  -glutamate following in vitro ischemia [ 5] is due to the absence of presynaptic glycine receptors leading to the inhibition.	transcription
53370	3	335024	5	NULL	NULL	0	NULL	glutamate	NULL		is released following	NULL				ischemia	NULL				NULL	in vitro	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_553_s_69	15020253	The present finding that in vitro ischemia induces glycine release with an extent  comparable to that of GABA release demonstrates that no involvement of glycine receptors  in inhibiting the release of  -glutamate following in vitro ischemia [ 5] is due to the absence of presynaptic glycine receptors leading to the inhibition.	transcription
53371	4	335024	5	NULL	NULL	0	NULL	glycine receptors	NULL		is not involved in	NULL				statement 3	NULL	inhibition of			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_553_s_69	15020253	The present finding that in vitro ischemia induces glycine release with an extent  comparable to that of GABA release demonstrates that no involvement of glycine receptors  in inhibiting the release of  -glutamate following in vitro ischemia [ 5] is due to the absence of presynaptic glycine receptors leading to the inhibition.	transcription
53372	5	335024	5	NULL	NULL	0	NULL	presynaptic glycine receptors	NULL	absence of	leads to	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_553_s_69	15020253	The present finding that in vitro ischemia induces glycine release with an extent  comparable to that of GABA release demonstrates that no involvement of glycine receptors  in inhibiting the release of  -glutamate following in vitro ischemia [ 5] is due to the absence of presynaptic glycine receptors leading to the inhibition.	transcription
53139	1	335024	7	NULL	NULL	0	NULL	in vitro ischemia	NULL		induce	NULL				glycine	NULL	release of			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_553_s_69	15020253	The present finding that in vitro ischemia induces glycine release with an extent  comparable to that of GABA release demonstrates that no involvement of glycine receptors  in inhibiting the release of  -glutamate following in vitro ischemia [ 5] is due to the absence of presynaptic glycine receptors leading to the inhibition.	transcription
53140	2	335024	7	NULL	NULL	0	NULL	in vitro ischemia	NULL		induce	NULL				GABA	NULL	release of			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_553_s_69	15020253	The present finding that in vitro ischemia induces glycine release with an extent  comparable to that of GABA release demonstrates that no involvement of glycine receptors  in inhibiting the release of  -glutamate following in vitro ischemia [ 5] is due to the absence of presynaptic glycine receptors leading to the inhibition.	transcription
53141	3	335024	7	NULL	NULL	0	NULL	in vitro ischemia	NULL		release	NULL				glutamate	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_553_s_69	15020253	The present finding that in vitro ischemia induces glycine release with an extent  comparable to that of GABA release demonstrates that no involvement of glycine receptors  in inhibiting the release of  -glutamate following in vitro ischemia [ 5] is due to the absence of presynaptic glycine receptors leading to the inhibition.	transcription
53142	4	335024	7	NULL	NULL	0	NULL	glycine receptors	NULL		is not involved in	NULL				statement 3	NULL	inhibition of			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_553_s_69	15020253	The present finding that in vitro ischemia induces glycine release with an extent  comparable to that of GABA release demonstrates that no involvement of glycine receptors  in inhibiting the release of  -glutamate following in vitro ischemia [ 5] is due to the absence of presynaptic glycine receptors leading to the inhibition.	transcription
53143	5	335024	7	NULL	NULL	0	NULL	statement 4	NULL		due to	NULL				presynaptic glycine receptors	NULL	absence of			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_553_s_69	15020253	The present finding that in vitro ischemia induces glycine release with an extent  comparable to that of GABA release demonstrates that no involvement of glycine receptors  in inhibiting the release of  -glutamate following in vitro ischemia [ 5] is due to the absence of presynaptic glycine receptors leading to the inhibition.	transcription
53144	6	335024	7	NULL	NULL	0	NULL	statement 1	NULL		demonstrate	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_553_s_69	15020253	The present finding that in vitro ischemia induces glycine release with an extent  comparable to that of GABA release demonstrates that no involvement of glycine receptors  in inhibiting the release of  -glutamate following in vitro ischemia [ 5] is due to the absence of presynaptic glycine receptors leading to the inhibition.	transcription
53145	7	335024	7	NULL	NULL	0	NULL	statement 2	NULL		demonstrate	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_553_s_69	15020253	The present finding that in vitro ischemia induces glycine release with an extent  comparable to that of GABA release demonstrates that no involvement of glycine receptors  in inhibiting the release of  -glutamate following in vitro ischemia [ 5] is due to the absence of presynaptic glycine receptors leading to the inhibition.	transcription
53374	1	335026	5	NULL	NULL	0	NULL	Zn2+	NULL		inhibits	NULL	competitively			glycine receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_96_6_3234_s_101	10077667	In contrast, 100 muM Zn2+ did not affect the maximum glycine responses, but it acted as a competitive inhibitor for glycine receptors, lowered the apparent glycine affinity, and shifted EC50 to the right (Fig.  5 B; EC50,Ctr = 40 muM, EC50,Zn2+ = 74 muM).	transcription
53375	2	335026	5	NULL	NULL	0	NULL	Zn2+	NULL		lowers	NULL				glycine	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw60_pnas_96_6_3234_s_101	10077667	In contrast, 100 muM Zn2+ did not affect the maximum glycine responses, but it acted as a competitive inhibitor for glycine receptors, lowered the apparent glycine affinity, and shifted EC50 to the right (Fig.  5 B; EC50,Ctr = 40 muM, EC50,Zn2+ = 74 muM).	transcription
53146	1	335026	7	NULL	NULL	0	NULL	Zn2+	NULL		inhibits	NULL	competitively			glycine receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_96_6_3234_s_101	10077667	In contrast, 100 muM Zn2+ did not affect the maximum glycine responses, but it acted as a competitive inhibitor for glycine receptors, lowered the apparent glycine affinity, and shifted EC50 to the right (Fig.  5 B; EC50,Ctr = 40 muM, EC50,Zn2+ = 74 muM).	transcription
53147	2	335026	7	NULL	NULL	0	NULL	Zn2+	NULL		lowers	NULL				glycine affinity	NULL				NULL		0	NULL	NULL	NULL	gw60_pnas_96_6_3234_s_101	10077667	In contrast, 100 muM Zn2+ did not affect the maximum glycine responses, but it acted as a competitive inhibitor for glycine receptors, lowered the apparent glycine affinity, and shifted EC50 to the right (Fig.  5 B; EC50,Ctr = 40 muM, EC50,Zn2+ = 74 muM).	transcription
53376	1	335027	5	NULL	NULL	0	NULL	trigonelline	NULL		inhibits	NULL				LTG59 strain	NULL	growth of			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_11_5647_s_124	12406761	The growth of strain LTG59 was inhibited by both 5 mM trigonelline and 5 mM triethylglycine in the presence of 100 muM glycine betaine (Table  2).	transcription
53377	2	335027	5	NULL	NULL	0	NULL	triethylglycine	NULL		inhibits	NULL				LTG59 strain	NULL	growth of			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_11_5647_s_124	12406761	The growth of strain LTG59 was inhibited by both 5 mM trigonelline and 5 mM triethylglycine in the presence of 100 muM glycine betaine (Table  2).	transcription
53378	3	335027	5	NULL	NULL	0	NULL	statement 1	NULL		in the presence of	NULL				glycine betaine	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_11_5647_s_124	12406761	The growth of strain LTG59 was inhibited by both 5 mM trigonelline and 5 mM triethylglycine in the presence of 100 muM glycine betaine (Table  2).	transcription
53379	4	335027	5	NULL	NULL	0	NULL	statement 2	NULL		in the presence of	NULL				glycine betaine	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_11_5647_s_124	12406761	The growth of strain LTG59 was inhibited by both 5 mM trigonelline and 5 mM triethylglycine in the presence of 100 muM glycine betaine (Table  2).	transcription
53148	1	335027	7	NULL	NULL	0	NULL	 trigonelline	NULL		inhibit	NULL				 LTG59	NULL	growth of			NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_68_11_5647_s_124	12406761	The growth of strain LTG59 was inhibited by both 5 mM trigonelline and 5 mM triethylglycine in the presence of 100 muM glycine betaine (Table  2).	transcription
53149	2	335027	7	NULL	NULL	0	NULL	triethylglycine	NULL		inhibit	NULL				LTG59	NULL	growth of			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_11_5647_s_124	12406761	The growth of strain LTG59 was inhibited by both 5 mM trigonelline and 5 mM triethylglycine in the presence of 100 muM glycine betaine (Table  2).	transcription
53150	3	335027	7	NULL	NULL	0	NULL	statement 1	NULL		in presence of	NULL				glycine betaine	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_11_5647_s_124	12406761	The growth of strain LTG59 was inhibited by both 5 mM trigonelline and 5 mM triethylglycine in the presence of 100 muM glycine betaine (Table  2).	transcription
53151	4	335027	7	NULL	NULL	0	NULL	statement 2	NULL		in presence of	NULL				glycine betaine	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_11_5647_s_124	12406761	The growth of strain LTG59 was inhibited by both 5 mM trigonelline and 5 mM triethylglycine in the presence of 100 muM glycine betaine (Table  2).	transcription
53380	1	335029	5	NULL	NULL	0	NULL	proQ220::Tn 5	NULL	insertion of	alters	NULL				proline porter II	NULL	regulation of			NULL	Escherichia coli	NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_26_1_49_s_1573	12007642	J.L. Milner and J.M. Wood, Insertion  proQ220::Tn 5 alters regulation of proline porter II, a transporter of proline and glycine betaine  in  Escherichia coli.	transcription
53381	2	335029	5	NULL	NULL	0	NULL	proline porter II	NULL		is a transporter of	NULL				proline	NULL				NULL	Escherichia coli	0	NULL	NULL	NULL	gw70_femsmicrobiolrev_26_1_49_s_1573	12007642	J.L. Milner and J.M. Wood, Insertion  proQ220::Tn 5 alters regulation of proline porter II, a transporter of proline and glycine betaine  in  Escherichia coli.	transcription
53382	3	335029	5	NULL	NULL	0	NULL	proline porter II	NULL		is a transporter of	NULL				glycine betaine	NULL				NULL	Escherichia coli	0	NULL	NULL	NULL	gw70_femsmicrobiolrev_26_1_49_s_1573	12007642	J.L. Milner and J.M. Wood, Insertion  proQ220::Tn 5 alters regulation of proline porter II, a transporter of proline and glycine betaine  in  Escherichia coli.	transcription
53152	1	335029	7	NULL	NULL	0	NULL	 proQ220::Tn 5	NULL		alters	NULL				proline porter II	NULL	regulation of			NULL	Escherichia coli	0	NULL	NULL	NULL	gw70_femsmicrobiolrev_26_1_49_s_1573	12007642	J.L. Milner and J.M. Wood, Insertion  proQ220::Tn 5 alters regulation of proline porter II, a transporter of proline and glycine betaine  in  Escherichia coli.	transcription
53153	2	335029	7	NULL	NULL	0	NULL	proline porter II	NULL		is a transporter of	NULL				proline	NULL				NULL	Escherichia coli	0	NULL	NULL	NULL	gw70_femsmicrobiolrev_26_1_49_s_1573	12007642	J.L. Milner and J.M. Wood, Insertion  proQ220::Tn 5 alters regulation of proline porter II, a transporter of proline and glycine betaine  in  Escherichia coli.	transcription
53154	3	335029	7	NULL	NULL	0	NULL	proline porter II	NULL		is a transporter of	NULL				glycine betaine 	NULL				NULL	Escherichia coli	0	NULL	NULL	NULL	gw70_femsmicrobiolrev_26_1_49_s_1573	12007642	J.L. Milner and J.M. Wood, Insertion  proQ220::Tn 5 alters regulation of proline porter II, a transporter of proline and glycine betaine  in  Escherichia coli.	transcription
53383	1	335032	5	NULL	NULL	0	NULL	TNFalpha	NULL	secretion of	is induced by	NULL				LPS	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_11_9435_s_137	12524422	Finally, LPS-induced TNFalpha secretion was significantly reduced with LCA, DCA, and CDCA and their taurine- or glycine-conjugated forms (Fig.  5 D).	transcription
53384	2	335032	5	NULL	NULL	0	NULL	LCA	NULL		reduces	NULL	significantly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_11_9435_s_137	12524422	Finally, LPS-induced TNFalpha secretion was significantly reduced with LCA, DCA, and CDCA and their taurine- or glycine-conjugated forms (Fig.  5 D).	transcription
53385	3	335032	5	NULL	NULL	0	NULL	DCA	NULL		reduces	NULL	significantly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_11_9435_s_137	12524422	Finally, LPS-induced TNFalpha secretion was significantly reduced with LCA, DCA, and CDCA and their taurine- or glycine-conjugated forms (Fig.  5 D).	transcription
53386	4	335032	5	NULL	NULL	0	NULL	CDCA	NULL		reduces	NULL	significantly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_11_9435_s_137	12524422	Finally, LPS-induced TNFalpha secretion was significantly reduced with LCA, DCA, and CDCA and their taurine- or glycine-conjugated forms (Fig.  5 D).	transcription
53387	5	335032	5	NULL	NULL	0	NULL	taurine-conjugated LCA	NULL		reduces	NULL	significantly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_11_9435_s_137	12524422	Finally, LPS-induced TNFalpha secretion was significantly reduced with LCA, DCA, and CDCA and their taurine- or glycine-conjugated forms (Fig.  5 D).	transcription
53388	6	335032	5	NULL	NULL	0	NULL	taurine-conjugated DCA	NULL		reduces	NULL	significantly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_11_9435_s_137	12524422	Finally, LPS-induced TNFalpha secretion was significantly reduced with LCA, DCA, and CDCA and their taurine- or glycine-conjugated forms (Fig.  5 D).	transcription
53389	7	335032	5	NULL	NULL	0	NULL	taurine-conjugated CDCA	NULL		reduces	NULL	significantly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_11_9435_s_137	12524422	Finally, LPS-induced TNFalpha secretion was significantly reduced with LCA, DCA, and CDCA and their taurine- or glycine-conjugated forms (Fig.  5 D).	transcription
53390	8	335032	5	NULL	NULL	0	NULL	glycine-conjugated LCA	NULL		reduces	NULL	significantly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_11_9435_s_137	12524422	Finally, LPS-induced TNFalpha secretion was significantly reduced with LCA, DCA, and CDCA and their taurine- or glycine-conjugated forms (Fig.  5 D).	transcription
53391	9	335032	5	NULL	NULL	0	NULL	glycine-conjugated DCA	NULL		reduces	NULL	significantly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_11_9435_s_137	12524422	Finally, LPS-induced TNFalpha secretion was significantly reduced with LCA, DCA, and CDCA and their taurine- or glycine-conjugated forms (Fig.  5 D).	transcription
53392	10	335032	5	NULL	NULL	0	NULL	glycine-conjugated CDCA	NULL		reduces	NULL	significantly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_11_9435_s_137	12524422	Finally, LPS-induced TNFalpha secretion was significantly reduced with LCA, DCA, and CDCA and their taurine- or glycine-conjugated forms (Fig.  5 D).	transcription
53393	11	335032	5	NULL	NULL	0	NULL	statement 5	NULL		is an alternative to	NULL				statement 8	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_11_9435_s_137	12524422	Finally, LPS-induced TNFalpha secretion was significantly reduced with LCA, DCA, and CDCA and their taurine- or glycine-conjugated forms (Fig.  5 D).	transcription
53394	12	335032	5	NULL	NULL	0	NULL	statement 6	NULL		is an alternative to	NULL				statement 9	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_11_9435_s_137	12524422	Finally, LPS-induced TNFalpha secretion was significantly reduced with LCA, DCA, and CDCA and their taurine- or glycine-conjugated forms (Fig.  5 D).	transcription
53395	13	335032	5	NULL	NULL	0	NULL	statement 7	NULL		is an alternative to	NULL				statement 10	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_11_9435_s_137	12524422	Finally, LPS-induced TNFalpha secretion was significantly reduced with LCA, DCA, and CDCA and their taurine- or glycine-conjugated forms (Fig.  5 D).	transcription
53155	1	335032	7	NULL	NULL	0	NULL	LPS	NULL		induce	NULL				TNFalpha 	NULL	secretion of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_11_9435_s_137	12524422	Finally, LPS-induced TNFalpha secretion was significantly reduced with LCA, DCA, and CDCA and their taurine- or glycine-conjugated forms (Fig.  5 D).	transcription
53156	2	335032	7	NULL	NULL	0	NULL	LCA	NULL		reduce	NULL	significantly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_11_9435_s_137	12524422	Finally, LPS-induced TNFalpha secretion was significantly reduced with LCA, DCA, and CDCA and their taurine- or glycine-conjugated forms (Fig.  5 D).	transcription
53157	3	335032	7	NULL	NULL	0	NULL	DCA	NULL		reduce	NULL	significantly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_11_9435_s_137	12524422	Finally, LPS-induced TNFalpha secretion was significantly reduced with LCA, DCA, and CDCA and their taurine- or glycine-conjugated forms (Fig.  5 D).	transcription
53158	4	335032	7	NULL	NULL	0	NULL	CDCA	NULL		reduce	NULL	significantly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_11_9435_s_137	12524422	Finally, LPS-induced TNFalpha secretion was significantly reduced with LCA, DCA, and CDCA and their taurine- or glycine-conjugated forms (Fig.  5 D).	transcription
53159	5	335032	7	NULL	NULL	0	NULL	taurine-conjugated form	NULL		reduce	NULL	significantly			statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_11_9435_s_137	12524422	Finally, LPS-induced TNFalpha secretion was significantly reduced with LCA, DCA, and CDCA and their taurine- or glycine-conjugated forms (Fig.  5 D).	transcription
53160	6	335032	7	NULL	NULL	0	NULL	glycine-conjugated form	NULL		reduce	NULL	significantly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_11_9435_s_137	12524422	Finally, LPS-induced TNFalpha secretion was significantly reduced with LCA, DCA, and CDCA and their taurine- or glycine-conjugated forms (Fig.  5 D).	transcription
53161	7	335032	7	NULL	NULL	0	NULL	statement 5	NULL		is an alternative to	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_11_9435_s_137	12524422	Finally, LPS-induced TNFalpha secretion was significantly reduced with LCA, DCA, and CDCA and their taurine- or glycine-conjugated forms (Fig.  5 D).	transcription
53396	1	335033	5	NULL	NULL	0	NULL	Apg10p	NULL		interacts with	NULL				Apg12p	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_41_39517_s_108	12890687	These results indicate that the interaction of Apg10p with Apg12p in the presence of Apg7p is dependent on the carboxyl-terminal glycine of Apg12p that is essential for the conjugation reaction ( Fig. 2 A,  lane 5).	transcription
53397	2	335033	5	NULL	NULL	0	NULL	statement 1	NULL		in the presence of	NULL				Apg7p	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_41_39517_s_108	12890687	These results indicate that the interaction of Apg10p with Apg12p in the presence of Apg7p is dependent on the carboxyl-terminal glycine of Apg12p that is essential for the conjugation reaction ( Fig. 2 A,  lane 5).	transcription
53398	3	335033	5	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				Apg12p	NULL		carboxyl-terminal glycine		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_41_39517_s_108	12890687	These results indicate that the interaction of Apg10p with Apg12p in the presence of Apg7p is dependent on the carboxyl-terminal glycine of Apg12p that is essential for the conjugation reaction ( Fig. 2 A,  lane 5).	transcription
53399	4	335033	5	NULL	NULL	0	NULL	Apg12p	NULL		is dependent on	NULL		carboxyl-terminal glycine		conjugation reaction	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_41_39517_s_108	12890687	These results indicate that the interaction of Apg10p with Apg12p in the presence of Apg7p is dependent on the carboxyl-terminal glycine of Apg12p that is essential for the conjugation reaction ( Fig. 2 A,  lane 5).	transcription
53162	1	335033	7	NULL	NULL	0	NULL	Apg10p	NULL		interacts with	NULL				Apg12p	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_41_39517_s_108	12890687	These results indicate that the interaction of Apg10p with Apg12p in the presence of Apg7p is dependent on the carboxyl-terminal glycine of Apg12p that is essential for the conjugation reaction ( Fig. 2 A,  lane 5).	transcription
53163	2	335033	7	NULL	NULL	0	NULL	statement 1	NULL		in presence of	NULL				Apg7p	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_41_39517_s_108	12890687	These results indicate that the interaction of Apg10p with Apg12p in the presence of Apg7p is dependent on the carboxyl-terminal glycine of Apg12p that is essential for the conjugation reaction ( Fig. 2 A,  lane 5).	transcription
53164	3	335033	7	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				Apg12p	NULL		 carboxyl-terminal glycine 		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_41_39517_s_108	12890687	These results indicate that the interaction of Apg10p with Apg12p in the presence of Apg7p is dependent on the carboxyl-terminal glycine of Apg12p that is essential for the conjugation reaction ( Fig. 2 A,  lane 5).	transcription
53165	4	335033	7	NULL	NULL	0	NULL	statement 3	NULL		essential for	NULL				conjugation reaction	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_41_39517_s_108	12890687	These results indicate that the interaction of Apg10p with Apg12p in the presence of Apg7p is dependent on the carboxyl-terminal glycine of Apg12p that is essential for the conjugation reaction ( Fig. 2 A,  lane 5).	transcription
53400	1	335034	5	NULL	NULL	0	NULL	A1	NULL		contains	NULL		UP1			NULL		RNA-binding domains		NULL		0	NULL	NULL	NULL	gw60_embo_18_7_1939_s_113	10202157	The N-terminal portion of A1 (called UP1) contains two RNA-binding domains but lacks the C-terminal glycine-rich domain (Figure  5).	transcription
53401	2	335034	5	NULL	NULL	0	NULL	A1	NULL		lacks	NULL		UP1			NULL		C-terminal glycine-rich domain		NULL		0	NULL	NULL	NULL	gw60_embo_18_7_1939_s_113	10202157	The N-terminal portion of A1 (called UP1) contains two RNA-binding domains but lacks the C-terminal glycine-rich domain (Figure  5).	transcription
53402	3	335034	5	NULL	NULL	0	NULL	UP1	NULL		is	NULL				N-terminal portion of A1	NULL				NULL		0	NULL	NULL	NULL	gw60_embo_18_7_1939_s_113	10202157	The N-terminal portion of A1 (called UP1) contains two RNA-binding domains but lacks the C-terminal glycine-rich domain (Figure  5).	transcription
53353	1	335034	7	NULL	NULL	0	NULL	A1	NULL		contains	NULL		N-terminal portion			NULL		two RNA-binding domains		NULL		0	NULL	NULL	NULL	gw60_embo_18_7_1939_s_113	10202157	The N-terminal portion of A1 (called UP1) contains two RNA-binding domains but lacks the C-terminal glycine-rich domain (Figure  5).	transcription
53354	2	335034	7	NULL	NULL	0	NULL	A1	NULL		lacks	NULL		N-terminal portion of 			NULL		C-terminal glycine-rich domain		NULL		0	NULL	NULL	NULL	gw60_embo_18_7_1939_s_113	10202157	The N-terminal portion of A1 (called UP1) contains two RNA-binding domains but lacks the C-terminal glycine-rich domain (Figure  5).	transcription
53355	3	335034	7	NULL	NULL	0	NULL	A1	NULL		is	NULL		N-terminal portion 		UP1	NULL	synonym of			NULL		0	NULL	NULL	NULL	gw60_embo_18_7_1939_s_113	10202157	The N-terminal portion of A1 (called UP1) contains two RNA-binding domains but lacks the C-terminal glycine-rich domain (Figure  5).	transcription
53403	1	335036	5	NULL	NULL	0	NULL	glycine	NULL		stimulates	NULL				spermatozoa	NULL	acrosomal exocytosis of;;human			NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_306_2_376_s_110	12804573	It is worth to mention that glycine stimulates acrosomal exocytosis of several mammalian spermatozoa including human, an effect blocked by strychnine [ 5,  6 and  10].	transcription
53404	2	335036	5	NULL	NULL	0	NULL	spermatozoa	NULL	acrosomal exocytosis of;;human	is blocked by	NULL				strychnine	NULL				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_306_2_376_s_110	12804573	It is worth to mention that glycine stimulates acrosomal exocytosis of several mammalian spermatozoa including human, an effect blocked by strychnine [ 5,  6 and  10].	transcription
53166	1	335036	7	NULL	NULL	0	NULL	glycine	NULL		stimulate	NULL				acrosomal exocytosis	NULL	human			NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_306_2_376_s_110	12804573	It is worth to mention that glycine stimulates acrosomal exocytosis of several mammalian spermatozoa including human, an effect blocked by strychnine [ 5,  6 and  10].	transcription
53167	2	335036	7	NULL	NULL	0	NULL	strychnine	NULL		blocks	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_306_2_376_s_110	12804573	It is worth to mention that glycine stimulates acrosomal exocytosis of several mammalian spermatozoa including human, an effect blocked by strychnine [ 5,  6 and  10].	transcription
53405	1	335037	5	NULL	NULL	0	NULL	TNFalpha mRNA	NULL	increase in	is caused by	NULL				Wy-14,643	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_176	9934846	Additionally, inactivation of Kupffer cells with either methyl palmitate or dietary glycine prevented the increase in TNFalpha mRNA caused by Wy-14,643 ( 4, 5).	transcription
53406	2	335037	5	NULL	NULL	0	NULL	Kupffer cells	NULL		is inactivated by	NULL				methyl palmitate	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_176	9934846	Additionally, inactivation of Kupffer cells with either methyl palmitate or dietary glycine prevented the increase in TNFalpha mRNA caused by Wy-14,643 ( 4, 5).	transcription
53407	3	335037	5	NULL	NULL	0	NULL	Kupffer cells	NULL		is inactivated by	NULL				glycine	NULL	dietary			NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_176	9934846	Additionally, inactivation of Kupffer cells with either methyl palmitate or dietary glycine prevented the increase in TNFalpha mRNA caused by Wy-14,643 ( 4, 5).	transcription
53408	4	335037	5	NULL	NULL	0	NULL	statement 2	NULL		is an alternative to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_176	9934846	Additionally, inactivation of Kupffer cells with either methyl palmitate or dietary glycine prevented the increase in TNFalpha mRNA caused by Wy-14,643 ( 4, 5).	transcription
53409	5	335037	5	NULL	NULL	0	NULL	statement 2	NULL		prevents	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_176	9934846	Additionally, inactivation of Kupffer cells with either methyl palmitate or dietary glycine prevented the increase in TNFalpha mRNA caused by Wy-14,643 ( 4, 5).	transcription
53410	6	335037	5	NULL	NULL	0	NULL	statement 3	NULL		prevents	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_176	9934846	Additionally, inactivation of Kupffer cells with either methyl palmitate or dietary glycine prevented the increase in TNFalpha mRNA caused by Wy-14,643 ( 4, 5).	transcription
53168	1	335037	7	NULL	NULL	0	NULL	Wy-14,643	NULL		increase	NULL				TNFalpha mRNA	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_176	9934846	Additionally, inactivation of Kupffer cells with either methyl palmitate or dietary glycine prevented the increase in TNFalpha mRNA caused by Wy-14,643 ( 4, 5).	transcription
53169	2	335037	7	NULL	NULL	0	NULL	Kupffer cells	NULL	 inactivation of 	prevents	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_176	9934846	Additionally, inactivation of Kupffer cells with either methyl palmitate or dietary glycine prevented the increase in TNFalpha mRNA caused by Wy-14,643 ( 4, 5).	transcription
53170	3	335037	7	NULL	NULL	0	NULL	statement 2	NULL		in presence of	NULL				methyl palmitate	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_176	9934846	Additionally, inactivation of Kupffer cells with either methyl palmitate or dietary glycine prevented the increase in TNFalpha mRNA caused by Wy-14,643 ( 4, 5).	transcription
53171	4	335037	7	NULL	NULL	0	NULL	statement 2	NULL		in presence of	NULL				dietary glycine	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_176	9934846	Additionally, inactivation of Kupffer cells with either methyl palmitate or dietary glycine prevented the increase in TNFalpha mRNA caused by Wy-14,643 ( 4, 5).	transcription
53172	5	335037	7	NULL	NULL	0	NULL	statement 3	NULL		is an alternative to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_176	9934846	Additionally, inactivation of Kupffer cells with either methyl palmitate or dietary glycine prevented the increase in TNFalpha mRNA caused by Wy-14,643 ( 4, 5).	transcription
53411	1	335038	5	NULL	NULL	0	NULL	hepatocyte	NULL	replication of	is induced by	NULL				Wy-14,643	NULL				NULL		NULL	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_194	9934846	In addition, dietary glycine has been shown to prevent Wy-14,643-induced hepatocyte replication by inhibiting Kupffer cell production of TNFalpha ( 5).	transcription
53412	2	335038	5	NULL	NULL	0	NULL	glycine	NULL	dietary	prevents	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_194	9934846	In addition, dietary glycine has been shown to prevent Wy-14,643-induced hepatocyte replication by inhibiting Kupffer cell production of TNFalpha ( 5).	transcription
53413	3	335038	5	NULL	NULL	0	NULL	Kupffer cell	NULL		is produced by	NULL				TNFalpha	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_194	9934846	In addition, dietary glycine has been shown to prevent Wy-14,643-induced hepatocyte replication by inhibiting Kupffer cell production of TNFalpha ( 5).	transcription
53414	4	335038	5	NULL	NULL	0	NULL	glycine	NULL	dietary	inhibits	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_194	9934846	In addition, dietary glycine has been shown to prevent Wy-14,643-induced hepatocyte replication by inhibiting Kupffer cell production of TNFalpha ( 5).	transcription
53415	5	335038	5	NULL	NULL	0	NULL	statement 4	NULL		leads to	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_194	9934846	In addition, dietary glycine has been shown to prevent Wy-14,643-induced hepatocyte replication by inhibiting Kupffer cell production of TNFalpha ( 5).	transcription
53173	1	335038	7	NULL	NULL	0	NULL	Wy-14,643	NULL		induce	NULL				 hepatocyte 	NULL	replication of			NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_194	9934846	In addition, dietary glycine has been shown to prevent Wy-14,643-induced hepatocyte replication by inhibiting Kupffer cell production of TNFalpha ( 5).	transcription
53174	2	335038	7	NULL	NULL	0	NULL	Kupffer cell 	NULL		produce	NULL				TNFalpha	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_194	9934846	In addition, dietary glycine has been shown to prevent Wy-14,643-induced hepatocyte replication by inhibiting Kupffer cell production of TNFalpha ( 5).	transcription
53175	3	335038	7	NULL	NULL	0	NULL	dietary glycine	NULL		prevent	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_194	9934846	In addition, dietary glycine has been shown to prevent Wy-14,643-induced hepatocyte replication by inhibiting Kupffer cell production of TNFalpha ( 5).	transcription
53176	4	335038	7	NULL	NULL	0	NULL	statement 3	NULL		occur by	NULL				statement 2	NULL	inhibition of			NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_20_1_27_s_194	9934846	In addition, dietary glycine has been shown to prevent Wy-14,643-induced hepatocyte replication by inhibiting Kupffer cell production of TNFalpha ( 5).	transcription
53416	1	335039	5	NULL	NULL	0	NULL	alanine	NULL		inhibit	NULL				GS enzymes	NULL	archaeal			NULL	Methanobacterium ivanovi	0	NULL	NULL	NULL	gw60_applenvironmicrob_67_10_4458_s_87	11571143	For comparison, 5 mM alanine or glycine inhibited the archaeal GS enzymes from  Methanobacterium ivanovi ( 2) and  A. fulgidus (H. Schreier, unpublished results) to a similar extent.	transcription
53417	2	335039	5	NULL	NULL	0	NULL	alanine	NULL		inhibit	NULL				GS enzymes	NULL	archaeal			NULL	A. fulgidus	0	NULL	NULL	NULL	gw60_applenvironmicrob_67_10_4458_s_87	11571143	For comparison, 5 mM alanine or glycine inhibited the archaeal GS enzymes from  Methanobacterium ivanovi ( 2) and  A. fulgidus (H. Schreier, unpublished results) to a similar extent.	transcription
53418	3	335039	5	NULL	NULL	0	NULL	glycine	NULL		inhibit	NULL				GS enzymes	NULL	archaeal			NULL	Methanobacterium ivanovi	0	NULL	NULL	NULL	gw60_applenvironmicrob_67_10_4458_s_87	11571143	For comparison, 5 mM alanine or glycine inhibited the archaeal GS enzymes from  Methanobacterium ivanovi ( 2) and  A. fulgidus (H. Schreier, unpublished results) to a similar extent.	transcription
53419	4	335039	5	NULL	NULL	0	NULL	glycine	NULL		inhibit	NULL				GS enzymes	NULL	archaeal			NULL	A. fulgidus	NULL	NULL	NULL	NULL	gw60_applenvironmicrob_67_10_4458_s_87	11571143	For comparison, 5 mM alanine or glycine inhibited the archaeal GS enzymes from  Methanobacterium ivanovi ( 2) and  A. fulgidus (H. Schreier, unpublished results) to a similar extent.	transcription
53420	5	335039	5	NULL	NULL	0	NULL	statement 1	NULL		is similar to	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_67_10_4458_s_87	11571143	For comparison, 5 mM alanine or glycine inhibited the archaeal GS enzymes from  Methanobacterium ivanovi ( 2) and  A. fulgidus (H. Schreier, unpublished results) to a similar extent.	transcription
53421	6	335039	5	NULL	NULL	0	NULL	statement 2	NULL		is similar to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_67_10_4458_s_87	11571143	For comparison, 5 mM alanine or glycine inhibited the archaeal GS enzymes from  Methanobacterium ivanovi ( 2) and  A. fulgidus (H. Schreier, unpublished results) to a similar extent.	transcription
53177	1	335039	7	NULL	NULL	0	NULL	alanine	NULL		inhibit	NULL				archaeal GS enzymes	NULL	Methanobacterium ivanovi 			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_67_10_4458_s_87	11571143	For comparison, 5 mM alanine or glycine inhibited the archaeal GS enzymes from  Methanobacterium ivanovi ( 2) and  A. fulgidus (H. Schreier, unpublished results) to a similar extent.	transcription
53178	2	335039	7	NULL	NULL	0	NULL	alanine	NULL		inhibit	NULL				 archaeal GS enzymes	NULL	A. fulgidus			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_67_10_4458_s_87	11571143	For comparison, 5 mM alanine or glycine inhibited the archaeal GS enzymes from  Methanobacterium ivanovi ( 2) and  A. fulgidus (H. Schreier, unpublished results) to a similar extent.	transcription
53179	3	335039	7	NULL	NULL	0	NULL	glycine	NULL		inhibit	NULL				archaeal GS enzymes	NULL	Methanobacterium ivanovi			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_67_10_4458_s_87	11571143	For comparison, 5 mM alanine or glycine inhibited the archaeal GS enzymes from  Methanobacterium ivanovi ( 2) and  A. fulgidus (H. Schreier, unpublished results) to a similar extent.	transcription
53180	4	335039	7	NULL	NULL	0	NULL	 glycine	NULL		inhibit	NULL				archaeal GS enzymes	NULL	A. fulgidus			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_67_10_4458_s_87	11571143	For comparison, 5 mM alanine or glycine inhibited the archaeal GS enzymes from  Methanobacterium ivanovi ( 2) and  A. fulgidus (H. Schreier, unpublished results) to a similar extent.	transcription
53181	5	335039	7	NULL	NULL	0	NULL	statement 1	NULL		is similar to	NULL				statement 2	NULL				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_67_10_4458_s_87	11571143	For comparison, 5 mM alanine or glycine inhibited the archaeal GS enzymes from  Methanobacterium ivanovi ( 2) and  A. fulgidus (H. Schreier, unpublished results) to a similar extent.	transcription
53182	6	335039	7	NULL	NULL	0	NULL	statement 3	NULL		is similar to	NULL				statement 4	NULL				NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_67_10_4458_s_87	11571143	For comparison, 5 mM alanine or glycine inhibited the archaeal GS enzymes from  Methanobacterium ivanovi ( 2) and  A. fulgidus (H. Schreier, unpublished results) to a similar extent.	transcription
53183	1	335041	7	NULL	NULL	0	NULL	glycine	NULL		mediates	NULL				current	NULL				NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_37_3_391_s_74	9681937	Colchicine inhibition of glycine mediated currents did not vary between oocytes maintained at room or cold temperatures ( n=5, Student's  t-test).	transcription
53184	2	335041	7	NULL	NULL	0	NULL	Colchicine	NULL		inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_37_3_391_s_74	9681937	Colchicine inhibition of glycine mediated currents did not vary between oocytes maintained at room or cold temperatures ( n=5, Student's  t-test).	transcription
53185	3	335041	7	NULL	NULL	0	NULL	statement 2	NULL		does not vary between	NULL				oocytes	NULL				NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_37_3_391_s_74	9681937	Colchicine inhibition of glycine mediated currents did not vary between oocytes maintained at room or cold temperatures ( n=5, Student's  t-test).	transcription
53422	1	335042	5	NULL	NULL	0	NULL	NFPS	NULL		abolishes	NULL	totally			glycine	NULL	effects of			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_41_1_88_s_117	11445189	In contrast, NFPS alone had no effect on [3] content, but the effects of glycine and sarcosine were totally abolished by 1  M NFPS ( Fig. 5).	transcription
53423	2	335042	5	NULL	NULL	0	NULL	NFPS	NULL		abolishes	NULL	totally			sarcosine	NULL	effects of			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_41_1_88_s_117	11445189	In contrast, NFPS alone had no effect on [3] content, but the effects of glycine and sarcosine were totally abolished by 1  M NFPS ( Fig. 5).	transcription
53186	1	335042	7	NULL	NULL	0	NULL	NFPS 	NULL		abolish	NULL	totally			 glycine	NULL	effect of			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_41_1_88_s_117	11445189	In contrast, NFPS alone had no effect on [3] content, but the effects of glycine and sarcosine were totally abolished by 1  M NFPS ( Fig. 5).	transcription
53187	2	335042	7	NULL	NULL	0	NULL	NFPS 	NULL		abolish	NULL	totally			sarcosine	NULL	effect of			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_41_1_88_s_117	11445189	In contrast, NFPS alone had no effect on [3] content, but the effects of glycine and sarcosine were totally abolished by 1  M NFPS ( Fig. 5).	transcription
53424	1	335043	5	NULL	NULL	0	NULL	synaptic events	NULL		is activated in	NULL				5 DIV neurons	NULL				NULL		0	NULL	NULL	NULL	gw60_neuroscience_108_3_493_s_168	11738262	The data shown in  Fig. 2 indicate that the synaptic events activated in 5 DIV neurons are mediated by glycine, GABAA, and, to a lesser extent, AMPA receptors.	transcription
53425	2	335043	5	NULL	NULL	0	NULL	glycine	NULL		mediates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_neuroscience_108_3_493_s_168	11738262	The data shown in  Fig. 2 indicate that the synaptic events activated in 5 DIV neurons are mediated by glycine, GABAA, and, to a lesser extent, AMPA receptors.	transcription
53426	3	335043	5	NULL	NULL	0	NULL	GABAA	NULL		mediates	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_108_3_493_s_168	11738262	The data shown in  Fig. 2 indicate that the synaptic events activated in 5 DIV neurons are mediated by glycine, GABAA, and, to a lesser extent, AMPA receptors.	transcription
53427	4	335043	5	NULL	NULL	0	NULL	AMPA receptors	NULL		mediates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_neuroscience_108_3_493_s_168	11738262	The data shown in  Fig. 2 indicate that the synaptic events activated in 5 DIV neurons are mediated by glycine, GABAA, and, to a lesser extent, AMPA receptors.	transcription
53194	1	335043	7	NULL	NULL	0	NULL	 glycine	NULL		mediates	NULL				synaptic events	NULL	activation of			NULL	DIV neurons	0	NULL	NULL	NULL	gw60_neuroscience_108_3_493_s_168	11738262	The data shown in  Fig. 2 indicate that the synaptic events activated in 5 DIV neurons are mediated by glycine, GABAA, and, to a lesser extent, AMPA receptors.	transcription
53195	2	335043	7	NULL	NULL	0	NULL	GABAA	NULL		mediates	NULL				synaptic events	NULL	activation of			NULL	DIV neurons	0	NULL	NULL	NULL	gw60_neuroscience_108_3_493_s_168	11738262	The data shown in  Fig. 2 indicate that the synaptic events activated in 5 DIV neurons are mediated by glycine, GABAA, and, to a lesser extent, AMPA receptors.	transcription
53196	3	335043	7	NULL	NULL	0	NULL	AMPA receptors	NULL		mediates	NULL				synaptic events	NULL	activation of			NULL	DIV neurons	NULL	NULL	NULL	NULL	gw60_neuroscience_108_3_493_s_168	11738262	The data shown in  Fig. 2 indicate that the synaptic events activated in 5 DIV neurons are mediated by glycine, GABAA, and, to a lesser extent, AMPA receptors.	transcription
53428	1	335045	5	NULL	NULL	0	NULL	Lsm4	NULL		interacts with	NULL	directly	carboxyl terminus		SMN	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_34_26370_s_167	10851237	The carboxyl terminus of Lsm4 contains an arginine-and glycine-rich domain that, when expressed on its own, is sufficient for direct interaction with SMN (Fig.  5 B).	transcription
53429	2	335045	5	NULL	NULL	0	NULL	Lsm4	NULL		contains	NULL		carboxyl terminus			NULL		glycine-rich domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_34_26370_s_167	10851237	The carboxyl terminus of Lsm4 contains an arginine-and glycine-rich domain that, when expressed on its own, is sufficient for direct interaction with SMN (Fig.  5 B).	transcription
53430	3	335045	5	NULL	NULL	0	NULL	Lsm4	NULL		contains	NULL		carboxyl terminus			NULL		arginine-rich domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_34_26370_s_167	10851237	The carboxyl terminus of Lsm4 contains an arginine-and glycine-rich domain that, when expressed on its own, is sufficient for direct interaction with SMN (Fig.  5 B).	transcription
53197	1	335045	7	NULL	NULL	0	NULL	Lsm4 	NULL		contains	NULL		carboxyl terminus			NULL		arginine-rich domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_34_26370_s_167	10851237	The carboxyl terminus of Lsm4 contains an arginine-and glycine-rich domain that, when expressed on its own, is sufficient for direct interaction with SMN (Fig.  5 B).	transcription
53198	2	335045	7	NULL	NULL	0	NULL	Lsm4	NULL		contains	NULL		carboxyl terminus			NULL		glycine-rich domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_34_26370_s_167	10851237	The carboxyl terminus of Lsm4 contains an arginine-and glycine-rich domain that, when expressed on its own, is sufficient for direct interaction with SMN (Fig.  5 B).	transcription
53199	3	335045	7	NULL	NULL	0	NULL	Lsm4	NULL		interacts with	NULL	directly	carboxyl terminus		SMN	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_34_26370_s_167	10851237	The carboxyl terminus of Lsm4 contains an arginine-and glycine-rich domain that, when expressed on its own, is sufficient for direct interaction with SMN (Fig.  5 B).	transcription
53200	4	335045	7	NULL	NULL	0	NULL	statement 1	NULL		is required for	NULL				statement 3	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_34_26370_s_167	10851237	The carboxyl terminus of Lsm4 contains an arginine-and glycine-rich domain that, when expressed on its own, is sufficient for direct interaction with SMN (Fig.  5 B).	transcription
53201	5	335045	7	NULL	NULL	0	NULL	statement 2	NULL		is required for	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_34_26370_s_167	10851237	The carboxyl terminus of Lsm4 contains an arginine-and glycine-rich domain that, when expressed on its own, is sufficient for direct interaction with SMN (Fig.  5 B).	transcription
53431	1	335047	5	NULL	NULL	0	NULL	Osteopontin	NULL		bind	NULL		RGD motif		alphavbeta3	NULL				NULL	surface of cells	NULL	NULL	NULL	NULL	gw60_jclininvest_98_10_2218_s_23	8941637	Osteopontin contains an arginine-glycine-aspartate  (RGD) motif which allows the molecule to bind to alphavbeta3 and  other integrins on the surface of cells ( 5,  6).	transcription
53432	2	335047	5	NULL	NULL	0	NULL	RGD	NULL		is	NULL				arginine-glycine-aspartate 	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_98_10_2218_s_23	8941637	Osteopontin contains an arginine-glycine-aspartate  (RGD) motif which allows the molecule to bind to alphavbeta3 and  other integrins on the surface of cells ( 5,  6).	transcription
53433	3	335047	5	NULL	NULL	0	NULL	Osteopontin	NULL		bind	NULL		RGD motif		integrins	NULL				NULL	surface of cells	0	NULL	NULL	NULL	gw60_jclininvest_98_10_2218_s_23	8941637	Osteopontin contains an arginine-glycine-aspartate  (RGD) motif which allows the molecule to bind to alphavbeta3 and  other integrins on the surface of cells ( 5,  6).	transcription
53202	1	335047	7	NULL	NULL	0	NULL	Osteopontin 	NULL		bind	NULL		RGD motif		alphavbeta3	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_98_10_2218_s_23	8941637	Osteopontin contains an arginine-glycine-aspartate  (RGD) motif which allows the molecule to bind to alphavbeta3 and  other integrins on the surface of cells ( 5,  6).	transcription
53203	2	335047	7	NULL	NULL	0	NULL	Osteopontin	NULL		bind	NULL		RGD motif		integrins	NULL				NULL	surface of cells	0	NULL	NULL	NULL	gw60_jclininvest_98_10_2218_s_23	8941637	Osteopontin contains an arginine-glycine-aspartate  (RGD) motif which allows the molecule to bind to alphavbeta3 and  other integrins on the surface of cells ( 5,  6).	transcription
53204	3	335047	7	NULL	NULL	0	NULL		NULL		is	NULL		RGD motif		arginine-glycine-aspartate	NULL				NULL		0	NULL	NULL	NULL	gw60_jclininvest_98_10_2218_s_23	8941637	Osteopontin contains an arginine-glycine-aspartate  (RGD) motif which allows the molecule to bind to alphavbeta3 and  other integrins on the surface of cells ( 5,  6).	transcription
53434	1	335049	5	NULL	NULL	0	NULL	SGAT	NULL		is	NULL				Serine-glyoxylate aminotransferase	NULL				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_biochemistry_44_48_16313196_s_2	16313196	Serine-glyoxylate aminotransferase (SGAT) from Hyphomicrobium methylovorum  is a pyridoxal 5''-phosphate (PLP) enzyme that catalyzes the interconversion  of l-serine and glyoxylate to hydroxypyruvate and glycine.	transcription
53435	2	335049	5	NULL	NULL	0	NULL	PLP	NULL		is	NULL				pyridoxal 5''-phosphate	NULL				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_biochemistry_44_48_16313196_s_2	16313196	Serine-glyoxylate aminotransferase (SGAT) from Hyphomicrobium methylovorum  is a pyridoxal 5''-phosphate (PLP) enzyme that catalyzes the interconversion  of l-serine and glyoxylate to hydroxypyruvate and glycine.	transcription
53436	3	335049	5	NULL	NULL	0	NULL	SGAT	NULL		is a type of	NULL				PLP enzyme	NULL				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_biochemistry_44_48_16313196_s_2	16313196	Serine-glyoxylate aminotransferase (SGAT) from Hyphomicrobium methylovorum  is a pyridoxal 5''-phosphate (PLP) enzyme that catalyzes the interconversion  of l-serine and glyoxylate to hydroxypyruvate and glycine.	transcription
53437	4	335049	5	NULL	NULL	0	NULL	l-serine	NULL		is converted to	NULL				hydroxypyruvate	NULL				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_biochemistry_44_48_16313196_s_2	16313196	Serine-glyoxylate aminotransferase (SGAT) from Hyphomicrobium methylovorum  is a pyridoxal 5''-phosphate (PLP) enzyme that catalyzes the interconversion  of l-serine and glyoxylate to hydroxypyruvate and glycine.	transcription
53438	5	335049	5	NULL	NULL	0	NULL	l-serine	NULL		is converted to	NULL				glycine	NULL				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_biochemistry_44_48_16313196_s_2	16313196	Serine-glyoxylate aminotransferase (SGAT) from Hyphomicrobium methylovorum  is a pyridoxal 5''-phosphate (PLP) enzyme that catalyzes the interconversion  of l-serine and glyoxylate to hydroxypyruvate and glycine.	transcription
53439	6	335049	5	NULL	NULL	0	NULL	glyoxylate	NULL		is converted to	NULL				hydroxypyruvate	NULL				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_biochemistry_44_48_16313196_s_2	16313196	Serine-glyoxylate aminotransferase (SGAT) from Hyphomicrobium methylovorum  is a pyridoxal 5''-phosphate (PLP) enzyme that catalyzes the interconversion  of l-serine and glyoxylate to hydroxypyruvate and glycine.	transcription
53440	7	335049	5	NULL	NULL	0	NULL	glyoxylate	NULL		is converted to	NULL				glycine	NULL				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_biochemistry_44_48_16313196_s_2	16313196	Serine-glyoxylate aminotransferase (SGAT) from Hyphomicrobium methylovorum  is a pyridoxal 5''-phosphate (PLP) enzyme that catalyzes the interconversion  of l-serine and glyoxylate to hydroxypyruvate and glycine.	transcription
53441	8	335049	5	NULL	NULL	0	NULL	statement 4	NULL		occurs along with	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_biochemistry_44_48_16313196_s_2	16313196	Serine-glyoxylate aminotransferase (SGAT) from Hyphomicrobium methylovorum  is a pyridoxal 5''-phosphate (PLP) enzyme that catalyzes the interconversion  of l-serine and glyoxylate to hydroxypyruvate and glycine.	transcription
53442	9	335049	5	NULL	NULL	0	NULL	statement 5	NULL		occurs along with	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_biochemistry_44_48_16313196_s_2	16313196	Serine-glyoxylate aminotransferase (SGAT) from Hyphomicrobium methylovorum  is a pyridoxal 5''-phosphate (PLP) enzyme that catalyzes the interconversion  of l-serine and glyoxylate to hydroxypyruvate and glycine.	transcription
53443	10	335049	5	NULL	NULL	0	NULL	statement 8	NULL		occurs along with	NULL				statement 9	NULL				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_biochemistry_44_48_16313196_s_2	16313196	Serine-glyoxylate aminotransferase (SGAT) from Hyphomicrobium methylovorum  is a pyridoxal 5''-phosphate (PLP) enzyme that catalyzes the interconversion  of l-serine and glyoxylate to hydroxypyruvate and glycine.	transcription
53444	11	335049	5	NULL	NULL	0	NULL	SGAT	NULL	Hyphomicrobium methylovorum	catalyzes	NULL				statement 10	NULL	interconversion of			NULL		0	NULL	NULL	NULL	abs-batch0540-0549_biochemistry_44_48_16313196_s_2	16313196	Serine-glyoxylate aminotransferase (SGAT) from Hyphomicrobium methylovorum  is a pyridoxal 5''-phosphate (PLP) enzyme that catalyzes the interconversion  of l-serine and glyoxylate to hydroxypyruvate and glycine.	transcription
53205	1	335049	7	NULL	NULL	0	NULL	 l-serine 	NULL		converted to	NULL				hydroxypyruvate	NULL				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_biochemistry_44_48_16313196_s_2	16313196	Serine-glyoxylate aminotransferase (SGAT) from Hyphomicrobium methylovorum  is a pyridoxal 5''-phosphate (PLP) enzyme that catalyzes the interconversion  of l-serine and glyoxylate to hydroxypyruvate and glycine.	transcription
53206	2	335049	7	NULL	NULL	0	NULL	l-serine	NULL		converted to	NULL				glycine	NULL				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_biochemistry_44_48_16313196_s_2	16313196	Serine-glyoxylate aminotransferase (SGAT) from Hyphomicrobium methylovorum  is a pyridoxal 5''-phosphate (PLP) enzyme that catalyzes the interconversion  of l-serine and glyoxylate to hydroxypyruvate and glycine.	transcription
53207	3	335049	7	NULL	NULL	0	NULL	glyoxylate	NULL		converted to	NULL				hydroxypyruvate	NULL				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_biochemistry_44_48_16313196_s_2	16313196	Serine-glyoxylate aminotransferase (SGAT) from Hyphomicrobium methylovorum  is a pyridoxal 5''-phosphate (PLP) enzyme that catalyzes the interconversion  of l-serine and glyoxylate to hydroxypyruvate and glycine.	transcription
53208	4	335049	7	NULL	NULL	0	NULL	glyoxylate	NULL		converted to	NULL				glycine	NULL				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_biochemistry_44_48_16313196_s_2	16313196	Serine-glyoxylate aminotransferase (SGAT) from Hyphomicrobium methylovorum  is a pyridoxal 5''-phosphate (PLP) enzyme that catalyzes the interconversion  of l-serine and glyoxylate to hydroxypyruvate and glycine.	transcription
53209	5	335049	7	NULL	NULL	0	NULL	statement 1	NULL		occur along with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_biochemistry_44_48_16313196_s_2	16313196	Serine-glyoxylate aminotransferase (SGAT) from Hyphomicrobium methylovorum  is a pyridoxal 5''-phosphate (PLP) enzyme that catalyzes the interconversion  of l-serine and glyoxylate to hydroxypyruvate and glycine.	transcription
53210	6	335049	7	NULL	NULL	0	NULL	statement 3	NULL		occur along with	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_biochemistry_44_48_16313196_s_2	16313196	Serine-glyoxylate aminotransferase (SGAT) from Hyphomicrobium methylovorum  is a pyridoxal 5''-phosphate (PLP) enzyme that catalyzes the interconversion  of l-serine and glyoxylate to hydroxypyruvate and glycine.	transcription
53211	7	335049	7	NULL	NULL	0	NULL	statement 5	NULL		occur along with	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_biochemistry_44_48_16313196_s_2	16313196	Serine-glyoxylate aminotransferase (SGAT) from Hyphomicrobium methylovorum  is a pyridoxal 5''-phosphate (PLP) enzyme that catalyzes the interconversion  of l-serine and glyoxylate to hydroxypyruvate and glycine.	transcription
53212	8	335049	7	NULL	NULL	0	NULL	SGAT	NULL	Hyphomicrobium methylovorum	catalyzes	NULL				statement 7	NULL	interconversion of			NULL		0	NULL	NULL	NULL	abs-batch0540-0549_biochemistry_44_48_16313196_s_2	16313196	Serine-glyoxylate aminotransferase (SGAT) from Hyphomicrobium methylovorum  is a pyridoxal 5''-phosphate (PLP) enzyme that catalyzes the interconversion  of l-serine and glyoxylate to hydroxypyruvate and glycine.	transcription
53213	9	335049	7	NULL	NULL	0	NULL	SGAT	NULL		is	NULL				Serine-glyoxylate aminotransferase	NULL				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_biochemistry_44_48_16313196_s_2	16313196	Serine-glyoxylate aminotransferase (SGAT) from Hyphomicrobium methylovorum  is a pyridoxal 5''-phosphate (PLP) enzyme that catalyzes the interconversion  of l-serine and glyoxylate to hydroxypyruvate and glycine.	transcription
53225	10	335049	7	NULL	NULL	0	NULL	SGAT	NULL		is a type of	NULL				PLP enzyme	NULL				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_biochemistry_44_48_16313196_s_2	16313196	Serine-glyoxylate aminotransferase (SGAT) from Hyphomicrobium methylovorum  is a pyridoxal 5''-phosphate (PLP) enzyme that catalyzes the interconversion  of l-serine and glyoxylate to hydroxypyruvate and glycine.	transcription
53226	11	335049	7	NULL	NULL	0	NULL	PLP	NULL		is	NULL				pyridoxal 5''-phosphate	NULL				NULL		NULL	NULL	NULL	NULL	abs-batch0540-0549_biochemistry_44_48_16313196_s_2	16313196	Serine-glyoxylate aminotransferase (SGAT) from Hyphomicrobium methylovorum  is a pyridoxal 5''-phosphate (PLP) enzyme that catalyzes the interconversion  of l-serine and glyoxylate to hydroxypyruvate and glycine.	transcription
53445	1	335052	5	NULL	NULL	0	NULL	lysine-56	NULL		bind	NULL	potentially			serine racemase	NULL		pyridoxal 5' phosphate		NULL		0	NULL	NULL	NULL	gw60_pnas_96_23_13409_s_93	10557334	To explore the dependence on pyridoxal 5' phosphate binding, we constructed a mutant in which lysine-56, predicted to bind pyridoxal 5' phosphate in serine racemase (Fig.  1 C), was replaced by glycine (K56G mutant).	transcription
53214	1	335052	7	NULL	NULL	0	NULL		NULL		bind	NULL	may	 lysine-56		serine racemase	NULL		pyridoxal 5' phosphate		NULL		0	NULL	NULL	NULL	gw60_pnas_96_23_13409_s_93	10557334	To explore the dependence on pyridoxal 5' phosphate binding, we constructed a mutant in which lysine-56, predicted to bind pyridoxal 5' phosphate in serine racemase (Fig.  1 C), was replaced by glycine (K56G mutant).	transcription
53446	1	335053	5	NULL	NULL	0	NULL	GlyR	NULL	WT	is inhibited by	NULL				PTX	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_43_35836_s_226	16109711	C, currents activated by 30 muM glycine in the WT GlyR are completely inhibited by 100 muM PTX ( left panel), whereas those activated by 5 muM glycine in the T6'F GlyR are little affected by 300 muM PTX ( center panel).	transcription
53447	2	335053	5	NULL	NULL	0	NULL	GlyR	NULL		is affected by	NULL	little	T6'F		PTX	NULL				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_43_35836_s_226	16109711	C, currents activated by 30 muM glycine in the WT GlyR are completely inhibited by 100 muM PTX ( left panel), whereas those activated by 5 muM glycine in the T6'F GlyR are little affected by 300 muM PTX ( center panel).	transcription
53215	1	335053	7	NULL	NULL	0	NULL	PTX	NULL		inhibit	NULL	completely			GlyR	NULL	WT			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_43_35836_s_226	16109711	C, currents activated by 30 muM glycine in the WT GlyR are completely inhibited by 100 muM PTX ( left panel), whereas those activated by 5 muM glycine in the T6'F GlyR are little affected by 300 muM PTX ( center panel).	transcription
53216	2	335053	7	NULL	NULL	0	NULL	PTX	NULL		affect	NULL	little			GlyR	NULL		T6'F		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_43_35836_s_226	16109711	C, currents activated by 30 muM glycine in the WT GlyR are completely inhibited by 100 muM PTX ( left panel), whereas those activated by 5 muM glycine in the T6'F GlyR are little affected by 300 muM PTX ( center panel).	transcription
53448	1	335054	5	NULL	NULL	0	NULL	glycine	NULL		is a type of	NULL				neurotransmitter	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_8_5_283_s_70	9501073	We were unable to demonstrate any rise in [Ca2+]i upon application of the neurotransmitter glycine ( n = 5), but currents induced by glycine were apparent in 20% of ganglion cell layer neurons ( n = 16), as recorded whole-cell patch-clamping (V.B., unpublished observation).	transcription
53449	2	335054	5	NULL	NULL	0	NULL	glycine	NULL	addition of	does not rise	NULL	potentially			[Ca2+]i	NULL				NULL		0	NULL	NULL	NULL	gw60_currbiol_8_5_283_s_70	9501073	We were unable to demonstrate any rise in [Ca2+]i upon application of the neurotransmitter glycine ( n = 5), but currents induced by glycine were apparent in 20% of ganglion cell layer neurons ( n = 16), as recorded whole-cell patch-clamping (V.B., unpublished observation).	transcription
53450	1	335055	5	NULL	NULL	0	NULL	spermine	NULL	stimulation of	is independent of	NULL				glycine	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_4_701_s_16	9380034	The glycine-independent form of spermine stimulation (Fig.  1A,  1), seen with saturating concentrations of glycine, may involve relief of proton inhibition (Fig.  1A,  6), processes that are also influenced by the alternatively spliced insert encoded by exon 5 in the NR1 subunit (Fig.  1A,  9).	transcription
53451	2	335055	5	NULL	NULL	0	NULL	statement 1	NULL		involves	NULL	may			proton	NULL	relief of;;inhibition of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_4_701_s_16	9380034	The glycine-independent form of spermine stimulation (Fig.  1A,  1), seen with saturating concentrations of glycine, may involve relief of proton inhibition (Fig.  1A,  6), processes that are also influenced by the alternatively spliced insert encoded by exon 5 in the NR1 subunit (Fig.  1A,  9).	transcription
53217	1	335055	7	NULL	NULL	0	NULL	spermine	NULL	stimulation of	is independent of	NULL				glycine	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_4_701_s_16	9380034	The glycine-independent form of spermine stimulation (Fig.  1A,  1), seen with saturating concentrations of glycine, may involve relief of proton inhibition (Fig.  1A,  6), processes that are also influenced by the alternatively spliced insert encoded by exon 5 in the NR1 subunit (Fig.  1A,  9).	transcription
53218	2	335055	7	NULL	NULL	0	NULL	statement 1	NULL		involve	NULL	may			proton inhibition	NULL	relief of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_4_701_s_16	9380034	The glycine-independent form of spermine stimulation (Fig.  1A,  1), seen with saturating concentrations of glycine, may involve relief of proton inhibition (Fig.  1A,  6), processes that are also influenced by the alternatively spliced insert encoded by exon 5 in the NR1 subunit (Fig.  1A,  9).	transcription
53219	3	335055	7	NULL	NULL	0	NULL	NR1 subunit 	NULL		influence	NULL			exon 5	proton inhibition	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_4_701_s_16	9380034	The glycine-independent form of spermine stimulation (Fig.  1A,  1), seen with saturating concentrations of glycine, may involve relief of proton inhibition (Fig.  1A,  6), processes that are also influenced by the alternatively spliced insert encoded by exon 5 in the NR1 subunit (Fig.  1A,  9).	transcription
53453	1	335056	5	NULL	NULL	0	NULL	glycine	NULL	concentration of	elevates within	NULL				synapse	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_58_1_129_s_209	10860934	The elevation in glycine concentrations within the synapse caused by pH inhibition of glycine transport may lead to increased activity of NMDA receptors containing the exon 5 in the NR-1 subunits and may be one of the factors triggering the subsequent destructive phase of ischemia.	transcription
53454	2	335056	5	NULL	NULL	0	NULL	glycine	NULL	transport of	is inhibited by	NULL				pH	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_58_1_129_s_209	10860934	The elevation in glycine concentrations within the synapse caused by pH inhibition of glycine transport may lead to increased activity of NMDA receptors containing the exon 5 in the NR-1 subunits and may be one of the factors triggering the subsequent destructive phase of ischemia.	transcription
53455	3	335056	5	NULL	NULL	0	NULL	statement 2	NULL		causes	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_58_1_129_s_209	10860934	The elevation in glycine concentrations within the synapse caused by pH inhibition of glycine transport may lead to increased activity of NMDA receptors containing the exon 5 in the NR-1 subunits and may be one of the factors triggering the subsequent destructive phase of ischemia.	transcription
53456	4	335056	5	NULL	NULL	0	NULL	NMDA receptors	NULL		contains	NULL					NULL		NR-1 subunits	exon 5	NULL		0	NULL	NULL	NULL	gw60_molpharmacol_58_1_129_s_209	10860934	The elevation in glycine concentrations within the synapse caused by pH inhibition of glycine transport may lead to increased activity of NMDA receptors containing the exon 5 in the NR-1 subunits and may be one of the factors triggering the subsequent destructive phase of ischemia.	transcription
53458	5	335056	5	NULL	NULL	0	NULL	statement 1	NULL		increases	NULL	may			statement 4	NULL	activity of			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_58_1_129_s_209	10860934	The elevation in glycine concentrations within the synapse caused by pH inhibition of glycine transport may lead to increased activity of NMDA receptors containing the exon 5 in the NR-1 subunits and may be one of the factors triggering the subsequent destructive phase of ischemia.	transcription
53459	6	335056	5	NULL	NULL	0	NULL	statement 1	NULL		triggers	NULL	may			ischemia	NULL	subsequent destructive phase of			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_58_1_129_s_209	10860934	The elevation in glycine concentrations within the synapse caused by pH inhibition of glycine transport may lead to increased activity of NMDA receptors containing the exon 5 in the NR-1 subunits and may be one of the factors triggering the subsequent destructive phase of ischemia.	transcription
53220	2	335056	7	NULL	NULL	0	NULL	statement 1	NULL		elevates	NULL				glycine	NULL	concentration of			NULL	within synapse	NULL	NULL	NULL	NULL	gw60_molpharmacol_58_1_129_s_209	10860934	The elevation in glycine concentrations within the synapse caused by pH inhibition of glycine transport may lead to increased activity of NMDA receptors containing the exon 5 in the NR-1 subunits and may be one of the factors triggering the subsequent destructive phase of ischemia.	transcription
53221	1	335056	7	NULL	NULL	0	NULL	glycine transport 	NULL		inhibited by	NULL				pH	NULL				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_58_1_129_s_209	10860934	The elevation in glycine concentrations within the synapse caused by pH inhibition of glycine transport may lead to increased activity of NMDA receptors containing the exon 5 in the NR-1 subunits and may be one of the factors triggering the subsequent destructive phase of ischemia.	transcription
53222	4	335056	7	NULL	NULL	0	NULL	statement 2	NULL		increase	NULL	may			statement 3	NULL	activity of			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_58_1_129_s_209	10860934	The elevation in glycine concentrations within the synapse caused by pH inhibition of glycine transport may lead to increased activity of NMDA receptors containing the exon 5 in the NR-1 subunits and may be one of the factors triggering the subsequent destructive phase of ischemia.	transcription
53223	3	335056	7	NULL	NULL	0	NULL	NMDA receptor	NULL		contain	NULL					NULL		NR-1 subunits 	exon 5	NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_58_1_129_s_209	10860934	The elevation in glycine concentrations within the synapse caused by pH inhibition of glycine transport may lead to increased activity of NMDA receptors containing the exon 5 in the NR-1 subunits and may be one of the factors triggering the subsequent destructive phase of ischemia.	transcription
53224	5	335056	7	NULL	NULL	0	NULL	statement 4	NULL		trigger	NULL	may			ischemia	NULL	destructive phase of			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_58_1_129_s_209	10860934	The elevation in glycine concentrations within the synapse caused by pH inhibition of glycine transport may lead to increased activity of NMDA receptors containing the exon 5 in the NR-1 subunits and may be one of the factors triggering the subsequent destructive phase of ischemia.	transcription
53460	1	335058	5	NULL	NULL	0	NULL	CPE	NULL	lower dose of	induce	NULL				DNA	NULL	cleavage of			NULL		0	NULL	NULL	NULL	gw70_infectimmun_71_8_4260_s_177	12874301	That lower CPE dose-induced DNA cleavage was blocked by a 50 muM concentration of the broad-spectrum caspase inhibitor Z-VAD-FMK but not by a 5 mM concentration of the oncosis inhibitor glycine (Fig.  3A).	transcription
53461	2	335058	5	NULL	NULL	0	NULL	Z-VAD-FMK	NULL		blocks	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_71_8_4260_s_177	12874301	That lower CPE dose-induced DNA cleavage was blocked by a 50 muM concentration of the broad-spectrum caspase inhibitor Z-VAD-FMK but not by a 5 mM concentration of the oncosis inhibitor glycine (Fig.  3A).	transcription
53462	3	335058	5	NULL	NULL	0	NULL	Z-VAD-FMK	NULL		is an inhibitor of	NULL				caspase	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_71_8_4260_s_177	12874301	That lower CPE dose-induced DNA cleavage was blocked by a 50 muM concentration of the broad-spectrum caspase inhibitor Z-VAD-FMK but not by a 5 mM concentration of the oncosis inhibitor glycine (Fig.  3A).	transcription
53463	4	335058	5	NULL	NULL	0	NULL	glycine	NULL		does not block	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_71_8_4260_s_177	12874301	That lower CPE dose-induced DNA cleavage was blocked by a 50 muM concentration of the broad-spectrum caspase inhibitor Z-VAD-FMK but not by a 5 mM concentration of the oncosis inhibitor glycine (Fig.  3A).	transcription
53464	5	335058	5	NULL	NULL	0	NULL	glycine	NULL		is an inhibitor of	NULL				oncosis	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_71_8_4260_s_177	12874301	That lower CPE dose-induced DNA cleavage was blocked by a 50 muM concentration of the broad-spectrum caspase inhibitor Z-VAD-FMK but not by a 5 mM concentration of the oncosis inhibitor glycine (Fig.  3A).	transcription
53227	1	335058	7	NULL	NULL	0	NULL	CPE	NULL		induce	NULL				DNA cleavage	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_71_8_4260_s_177	12874301	That lower CPE dose-induced DNA cleavage was blocked by a 50 muM concentration of the broad-spectrum caspase inhibitor Z-VAD-FMK but not by a 5 mM concentration of the oncosis inhibitor glycine (Fig.  3A).	transcription
53228	2	335058	7	NULL	NULL	0	NULL	Z-VAD-FMK	NULL		inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_71_8_4260_s_177	12874301	That lower CPE dose-induced DNA cleavage was blocked by a 50 muM concentration of the broad-spectrum caspase inhibitor Z-VAD-FMK but not by a 5 mM concentration of the oncosis inhibitor glycine (Fig.  3A).	transcription
53229	3	335058	7	NULL	NULL	0	NULL	Z-VAD-FMK	NULL		is a type of	NULL				broad-spectrum caspase inhibitor	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_71_8_4260_s_177	12874301	That lower CPE dose-induced DNA cleavage was blocked by a 50 muM concentration of the broad-spectrum caspase inhibitor Z-VAD-FMK but not by a 5 mM concentration of the oncosis inhibitor glycine (Fig.  3A).	transcription
53230	4	335058	7	NULL	NULL	0	NULL	glycine	NULL		does not inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_71_8_4260_s_177	12874301	That lower CPE dose-induced DNA cleavage was blocked by a 50 muM concentration of the broad-spectrum caspase inhibitor Z-VAD-FMK but not by a 5 mM concentration of the oncosis inhibitor glycine (Fig.  3A).	transcription
53231	5	335058	7	NULL	NULL	0	NULL	glycine	NULL		is a type of	NULL				oncosis inhibitor	NULL				NULL		0	NULL	NULL	NULL	gw70_infectimmun_71_8_4260_s_177	12874301	That lower CPE dose-induced DNA cleavage was blocked by a 50 muM concentration of the broad-spectrum caspase inhibitor Z-VAD-FMK but not by a 5 mM concentration of the oncosis inhibitor glycine (Fig.  3A).	transcription
53483	1	335059	5	NULL	NULL	0	NULL	tetrahydrofolate-responsive protein	NULL		bind	NULL					NULL			glycine regulatory region	NULL		0	NULL	NULL	NULL	gw70_annurevplantbiol_52_0_119_s_479	null	Control of expression of  one-carbon metabolism genes of  Saccharomyces cerevisiae is mediated by a tetrahydrofolate-responsive protein binding to a glycine regulatory  region including a core 5''-CTTCTT-3'' motif.	transcription
53484	2	335059	5	NULL	NULL	0	NULL	glycine regulatory region	NULL		includes	NULL					NULL			core 5''-CTTCTT-3'' motif	NULL		0	NULL	NULL	NULL	gw70_annurevplantbiol_52_0_119_s_479	null	Control of expression of  one-carbon metabolism genes of  Saccharomyces cerevisiae is mediated by a tetrahydrofolate-responsive protein binding to a glycine regulatory  region including a core 5''-CTTCTT-3'' motif.	transcription
53485	3	335059	5	NULL	NULL	0	NULL	statement 1	NULL		mediate	NULL				one-carbon metabolism genes	NULL	control of;;expression of;;Saccharomyces cerevisiae			NULL		0	NULL	NULL	NULL	gw70_annurevplantbiol_52_0_119_s_479	null	Control of expression of  one-carbon metabolism genes of  Saccharomyces cerevisiae is mediated by a tetrahydrofolate-responsive protein binding to a glycine regulatory  region including a core 5''-CTTCTT-3'' motif.	transcription
53232	1	335059	7	NULL	NULL	0	NULL	tetrahydrofolate-responsive protein	NULL		bind	NULL					NULL		glycine regulatory region		NULL		0	NULL	NULL	NULL	gw70_annurevplantbiol_52_0_119_s_479	null	Control of expression of  one-carbon metabolism genes of  Saccharomyces cerevisiae is mediated by a tetrahydrofolate-responsive protein binding to a glycine regulatory  region including a core 5''-CTTCTT-3'' motif.	transcription
53233	2	335059	7	NULL	NULL	0	NULL	glycine regulatory region	NULL		include	NULL					NULL		core 5''-CTTCTT-3'' motif		NULL		0	NULL	NULL	NULL	gw70_annurevplantbiol_52_0_119_s_479	null	Control of expression of  one-carbon metabolism genes of  Saccharomyces cerevisiae is mediated by a tetrahydrofolate-responsive protein binding to a glycine regulatory  region including a core 5''-CTTCTT-3'' motif.	transcription
53234	3	335059	7	NULL	NULL	0	NULL	tetrahydrofolate-responsive protein	NULL		mediate	NULL				one-carbon metabolism genes	NULL	expression of;;Saccharomyces cerevisiae			NULL		0	NULL	NULL	NULL	gw70_annurevplantbiol_52_0_119_s_479	null	Control of expression of  one-carbon metabolism genes of  Saccharomyces cerevisiae is mediated by a tetrahydrofolate-responsive protein binding to a glycine regulatory  region including a core 5''-CTTCTT-3'' motif.	transcription
53235	1	335060	7	NULL	NULL	0	NULL	ApoL-I	NULL		bind	NULL				anti-apoL-I	NULL				NULL		0	NULL	NULL	NULL	gw70_nature_422_6927_83_s_131	12621437	ApoL-I was obtained by elution of the NHS material bound to anti-apoL-I-Sepharose,  using 5% CHAPS, 0.1 M glycine (pH 2.8) followed by neutralization with 1 M Tris (pH  8.0).	transcription
53486	1	335061	5	NULL	NULL	0	NULL	glycine	NULL		induces	NULL				Cl currents	NULL				NULL		0	NULL	NULL	NULL	gw70_neuropharmacology_51_4_701_s_42	16842826	Glycine-induced Cl  currents were low-pass filtered at 5 kHz, monitored on an oscilloscope and a chart  recorder (Gould TA240), and stored on a computer (pClamp 6.0, Axon Instruments) for  subsequent analysis.	transcription
53236	1	335061	7	NULL	NULL	0	NULL	Glycine	NULL		induce	NULL				Cl currents 	NULL				NULL		0	NULL	NULL	NULL	gw70_neuropharmacology_51_4_701_s_42	16842826	Glycine-induced Cl  currents were low-pass filtered at 5 kHz, monitored on an oscilloscope and a chart  recorder (Gould TA240), and stored on a computer (pClamp 6.0, Axon Instruments) for  subsequent analysis.	transcription
53487	1	335062	5	NULL	NULL	0	NULL		NULL		is substituted for	NULL		octarepeat histidine residues			NULL		glycine (PHGG(G/S)WGQ4 PGGG(G/S)WGQ4) 		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_53_55443_s_217	15459186	Missense mutations substituting octarepeat histidine residues for glycine (PHGG(G/S)WGQ4   PGGG(G/S)WGQ4) also inactivated the protective effect of PrPC ( Fig. 5).	transcription
53488	2	335062	5	NULL	NULL	0	NULL	statement 1	NULL		inactivates	NULL				PrPC	NULL	protective effect of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_53_55443_s_217	15459186	Missense mutations substituting octarepeat histidine residues for glycine (PHGG(G/S)WGQ4   PGGG(G/S)WGQ4) also inactivated the protective effect of PrPC ( Fig. 5).	transcription
53237	1	335062	7	NULL	NULL	0	NULL		NULL	Missense mutant	substituted for	NULL		octarepeat histidine residues			NULL		 glycine		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_53_55443_s_217	15459186	Missense mutations substituting octarepeat histidine residues for glycine (PHGG(G/S)WGQ4   PGGG(G/S)WGQ4) also inactivated the protective effect of PrPC ( Fig. 5).	transcription
53238	3	335062	7	NULL	NULL	0	NULL	statement 1	NULL		inactivate	NULL				PrPC	NULL	protective effect of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_53_55443_s_217	15459186	Missense mutations substituting octarepeat histidine residues for glycine (PHGG(G/S)WGQ4   PGGG(G/S)WGQ4) also inactivated the protective effect of PrPC ( Fig. 5).	transcription
53239	2	335062	7	NULL	NULL	0	NULL	statement 1	NULL		contains	NULL					NULL		(PHGG(G/S)WGQ4 PGGG(G/S)WGQ4)		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_53_55443_s_217	15459186	Missense mutations substituting octarepeat histidine residues for glycine (PHGG(G/S)WGQ4   PGGG(G/S)WGQ4) also inactivated the protective effect of PrPC ( Fig. 5).	transcription
53489	1	335063	5	NULL	NULL	0	NULL	NE	NULL		is relased from	NULL				hippocampal synaptosomes	NULL				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_313_1_242_s_115	15608072	As shown in  Fig. 2, addition to the superfusion medium of PP2 (1 muM) or lavendustin A (5 muM) inhibited in part the [3]NE release induced by SRIF-14/NMDA/glycine from hippocampal synaptosomes.	transcription
53490	2	335063	5	NULL	NULL	0	NULL	SRIF-14/NMDA/glycine	NULL		induces	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_313_1_242_s_115	15608072	As shown in  Fig. 2, addition to the superfusion medium of PP2 (1 muM) or lavendustin A (5 muM) inhibited in part the [3]NE release induced by SRIF-14/NMDA/glycine from hippocampal synaptosomes.	transcription
53491	3	335063	5	NULL	NULL	0	NULL	PP2	NULL		inhibits	NULL	partly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_313_1_242_s_115	15608072	As shown in  Fig. 2, addition to the superfusion medium of PP2 (1 muM) or lavendustin A (5 muM) inhibited in part the [3]NE release induced by SRIF-14/NMDA/glycine from hippocampal synaptosomes.	transcription
53492	4	335063	5	NULL	NULL	0	NULL	lavendustin A	NULL		inhibits	NULL	partly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_313_1_242_s_115	15608072	As shown in  Fig. 2, addition to the superfusion medium of PP2 (1 muM) or lavendustin A (5 muM) inhibited in part the [3]NE release induced by SRIF-14/NMDA/glycine from hippocampal synaptosomes.	transcription
53493	5	335063	5	NULL	NULL	0	NULL	statement 3	NULL		is an alternative to	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_313_1_242_s_115	15608072	As shown in  Fig. 2, addition to the superfusion medium of PP2 (1 muM) or lavendustin A (5 muM) inhibited in part the [3]NE release induced by SRIF-14/NMDA/glycine from hippocampal synaptosomes.	transcription
53240	1	335063	7	NULL	NULL	0	NULL	SRIF-14/NMDA/glycine	NULL	 hippocampal synaptosomes	induce	NULL				NE	NULL	release of			NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_313_1_242_s_115	15608072	As shown in  Fig. 2, addition to the superfusion medium of PP2 (1 muM) or lavendustin A (5 muM) inhibited in part the [3]NE release induced by SRIF-14/NMDA/glycine from hippocampal synaptosomes.	transcription
53241	2	335063	7	NULL	NULL	0	NULL	 PP2 	NULL		inhibit	NULL	partly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_313_1_242_s_115	15608072	As shown in  Fig. 2, addition to the superfusion medium of PP2 (1 muM) or lavendustin A (5 muM) inhibited in part the [3]NE release induced by SRIF-14/NMDA/glycine from hippocampal synaptosomes.	transcription
53242	3	335063	7	NULL	NULL	0	NULL	 lavendustin A	NULL		inhibit	NULL	partly			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_313_1_242_s_115	15608072	As shown in  Fig. 2, addition to the superfusion medium of PP2 (1 muM) or lavendustin A (5 muM) inhibited in part the [3]NE release induced by SRIF-14/NMDA/glycine from hippocampal synaptosomes.	transcription
53494	1	335064	5	NULL	NULL	0	NULL	ETC	NULL		is	NULL				electron transport chain	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_412_2_265_s_8	9256232	It was shown that oxidation of glycine coupled with NADH oxidation in mitochondrial electron transport chain (ETC) is less inhibited by the inhibitor of Complex I rotenone than oxidation of other mitochondrial substrates  [ 5.	transcription
53495	2	335064	5	NULL	NULL	0	NULL	glycine	NULL	oxidation of	is coupled with	NULL				NADH	NULL	oxidation of			NULL	mitochondrial ETC	0	NULL	NULL	NULL	gw60_febslett_412_2_265_s_8	9256232	It was shown that oxidation of glycine coupled with NADH oxidation in mitochondrial electron transport chain (ETC) is less inhibited by the inhibitor of Complex I rotenone than oxidation of other mitochondrial substrates  [ 5.	transcription
53496	3	335064	5	NULL	NULL	0	NULL	rotenone	NULL		is an inhibitor of	NULL				Complex I	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_412_2_265_s_8	9256232	It was shown that oxidation of glycine coupled with NADH oxidation in mitochondrial electron transport chain (ETC) is less inhibited by the inhibitor of Complex I rotenone than oxidation of other mitochondrial substrates  [ 5.	transcription
53497	4	335064	5	NULL	NULL	0	NULL	rotenone	NULL		inhibits	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_412_2_265_s_8	9256232	It was shown that oxidation of glycine coupled with NADH oxidation in mitochondrial electron transport chain (ETC) is less inhibited by the inhibitor of Complex I rotenone than oxidation of other mitochondrial substrates  [ 5.	transcription
53498	5	335064	5	NULL	NULL	0	NULL	rotenone	NULL		inhibits	NULL				substrates	NULL	oxidation of;;mitochondrial			NULL		0	NULL	NULL	NULL	gw60_febslett_412_2_265_s_8	9256232	It was shown that oxidation of glycine coupled with NADH oxidation in mitochondrial electron transport chain (ETC) is less inhibited by the inhibitor of Complex I rotenone than oxidation of other mitochondrial substrates  [ 5.	transcription
53499	6	335064	5	NULL	NULL	0	NULL	statement 4	NULL		lesser than	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_412_2_265_s_8	9256232	It was shown that oxidation of glycine coupled with NADH oxidation in mitochondrial electron transport chain (ETC) is less inhibited by the inhibitor of Complex I rotenone than oxidation of other mitochondrial substrates  [ 5.	transcription
53243	1	335064	7	NULL	NULL	0	NULL	glycine 	NULL	oxidation of	coupled with	NULL				NADH	NULL	oxidation of			NULL	mitochondrial ETC	NULL	NULL	NULL	NULL	gw60_febslett_412_2_265_s_8	9256232	It was shown that oxidation of glycine coupled with NADH oxidation in mitochondrial electron transport chain (ETC) is less inhibited by the inhibitor of Complex I rotenone than oxidation of other mitochondrial substrates  [ 5.	transcription
53270	2	335064	7	NULL	NULL	0	NULL	Complex I rotenone	NULL	inhibitor of	inhibit	NULL				statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw60_febslett_412_2_265_s_8	9256232	It was shown that oxidation of glycine coupled with NADH oxidation in mitochondrial electron transport chain (ETC) is less inhibited by the inhibitor of Complex I rotenone than oxidation of other mitochondrial substrates  [ 5.	transcription
53271	3	335064	7	NULL	NULL	0	NULL	substrates	NULL	oxidation of;;mitochondrial	inhibit	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_412_2_265_s_8	9256232	It was shown that oxidation of glycine coupled with NADH oxidation in mitochondrial electron transport chain (ETC) is less inhibited by the inhibitor of Complex I rotenone than oxidation of other mitochondrial substrates  [ 5.	transcription
53272	4	335064	7	NULL	NULL	0	NULL	statement 2	NULL	inhibition of	is less than	NULL				statement 3	NULL	inhibition of			NULL		NULL	NULL	NULL	NULL	gw60_febslett_412_2_265_s_8	9256232	It was shown that oxidation of glycine coupled with NADH oxidation in mitochondrial electron transport chain (ETC) is less inhibited by the inhibitor of Complex I rotenone than oxidation of other mitochondrial substrates  [ 5.	transcription
53273	5	335064	7	NULL	NULL	0	NULL	ETC	NULL		is	NULL				electron transport chain	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_412_2_265_s_8	9256232	It was shown that oxidation of glycine coupled with NADH oxidation in mitochondrial electron transport chain (ETC) is less inhibited by the inhibitor of Complex I rotenone than oxidation of other mitochondrial substrates  [ 5.	transcription
53500	1	335065	5	NULL	NULL	0	NULL	Class III ribonucleotide reductase	NULL		catalyzes	NULL				AdoMet	NULL	reductive cleavage of			NULL		0	NULL	NULL	NULL	gw60_febslett_529_2_237_s_183	12372607	Class III ribonucleotide reductase also catalyzes reductive cleavage of AdoMet to generate 5''-deoxyadenosine, in this case as an oxidant for a polypeptide glycine residue, generating a glycyl radical that is required for initiating ribonucleotide reduction [  38].	transcription
53501	2	335065	5	NULL	NULL	0	NULL	statement 1	NULL		generates	NULL				5''-deoxyadenosine	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_529_2_237_s_183	12372607	Class III ribonucleotide reductase also catalyzes reductive cleavage of AdoMet to generate 5''-deoxyadenosine, in this case as an oxidant for a polypeptide glycine residue, generating a glycyl radical that is required for initiating ribonucleotide reduction [  38].	transcription
53502	3	335065	5	NULL	NULL	0	NULL	Class III ribonucleotide reductase	NULL		acts as	NULL				polypeptide glycine residue	NULL	oxidant for			NULL		0	NULL	NULL	NULL	gw60_febslett_529_2_237_s_183	12372607	Class III ribonucleotide reductase also catalyzes reductive cleavage of AdoMet to generate 5''-deoxyadenosine, in this case as an oxidant for a polypeptide glycine residue, generating a glycyl radical that is required for initiating ribonucleotide reduction [  38].	transcription
53503	4	335065	5	NULL	NULL	0	NULL	statement 3	NULL		generates	NULL				glycyl radical	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_529_2_237_s_183	12372607	Class III ribonucleotide reductase also catalyzes reductive cleavage of AdoMet to generate 5''-deoxyadenosine, in this case as an oxidant for a polypeptide glycine residue, generating a glycyl radical that is required for initiating ribonucleotide reduction [  38].	transcription
53504	5	335065	5	NULL	NULL	0	NULL	glycyl radical	NULL		is required for	NULL				ribonucleotide	NULL	initiating;;reduction of			NULL		NULL	NULL	NULL	NULL	gw60_febslett_529_2_237_s_183	12372607	Class III ribonucleotide reductase also catalyzes reductive cleavage of AdoMet to generate 5''-deoxyadenosine, in this case as an oxidant for a polypeptide glycine residue, generating a glycyl radical that is required for initiating ribonucleotide reduction [  38].	transcription
53274	1	335065	7	NULL	NULL	0	NULL	Class III ribonucleotide reductase	NULL		catalyse	NULL				AdoMet	NULL	 reductive cleavage of 			NULL		0	NULL	NULL	NULL	gw60_febslett_529_2_237_s_183	12372607	Class III ribonucleotide reductase also catalyzes reductive cleavage of AdoMet to generate 5''-deoxyadenosine, in this case as an oxidant for a polypeptide glycine residue, generating a glycyl radical that is required for initiating ribonucleotide reduction [  38].	transcription
53275	2	335065	7	NULL	NULL	0	NULL	statement 1	NULL		generate	NULL				5''-deoxyadenosine	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_529_2_237_s_183	12372607	Class III ribonucleotide reductase also catalyzes reductive cleavage of AdoMet to generate 5''-deoxyadenosine, in this case as an oxidant for a polypeptide glycine residue, generating a glycyl radical that is required for initiating ribonucleotide reduction [  38].	transcription
53276	3	335065	7	NULL	NULL	0	NULL	Class III ribonucleotide reductase	NULL		generates	NULL				glycyl radical	NULL				NULL		0	NULL	NULL	NULL	gw60_febslett_529_2_237_s_183	12372607	Class III ribonucleotide reductase also catalyzes reductive cleavage of AdoMet to generate 5''-deoxyadenosine, in this case as an oxidant for a polypeptide glycine residue, generating a glycyl radical that is required for initiating ribonucleotide reduction [  38].	transcription
53277	4	335065	7	NULL	NULL	0	NULL	Class III ribonucleotide reductase	NULL		acts as a 	NULL				polypeptide glycine residue	NULL	oxidant for			NULL		0	NULL	NULL	NULL	gw60_febslett_529_2_237_s_183	12372607	Class III ribonucleotide reductase also catalyzes reductive cleavage of AdoMet to generate 5''-deoxyadenosine, in this case as an oxidant for a polypeptide glycine residue, generating a glycyl radical that is required for initiating ribonucleotide reduction [  38].	transcription
53278	5	335065	7	NULL	NULL	0	NULL	statement 3	NULL		is required for	NULL				ribonucleotide	NULL	initiating;;  reduction of			NULL		0	NULL	NULL	NULL	gw60_febslett_529_2_237_s_183	12372607	Class III ribonucleotide reductase also catalyzes reductive cleavage of AdoMet to generate 5''-deoxyadenosine, in this case as an oxidant for a polypeptide glycine residue, generating a glycyl radical that is required for initiating ribonucleotide reduction [  38].	transcription
53505	1	335067	5	NULL	NULL	0	NULL	MPO	NULL		induce	NULL				LDL	NULL	modification of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1481_1_109_s_167	11004581	Methionine showed an even stronger retarding effect on MPO-induced LDL modification among the HOCl traps used (factor 103), while glycine was the least effective (factor 13,  Fig. 5).	transcription
53506	2	335067	5	NULL	NULL	0	NULL	methionine	NULL		retard	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1481_1_109_s_167	11004581	Methionine showed an even stronger retarding effect on MPO-induced LDL modification among the HOCl traps used (factor 103), while glycine was the least effective (factor 13,  Fig. 5).	transcription
53507	3	335067	5	NULL	NULL	0	NULL	glycine	NULL		retard	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1481_1_109_s_167	11004581	Methionine showed an even stronger retarding effect on MPO-induced LDL modification among the HOCl traps used (factor 103), while glycine was the least effective (factor 13,  Fig. 5).	transcription
53508	4	335067	5	NULL	NULL	0	NULL	statement 2	NULL		stronger than	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1481_1_109_s_167	11004581	Methionine showed an even stronger retarding effect on MPO-induced LDL modification among the HOCl traps used (factor 103), while glycine was the least effective (factor 13,  Fig. 5).	transcription
53279	1	335067	7	NULL	NULL	0	NULL	MPO	NULL		induce	NULL				LDL	NULL	modification of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1481_1_109_s_167	11004581	Methionine showed an even stronger retarding effect on MPO-induced LDL modification among the HOCl traps used (factor 103), while glycine was the least effective (factor 13,  Fig. 5).	transcription
53280	2	335067	7	NULL	NULL	0	NULL	Methionine	NULL		retard	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1481_1_109_s_167	11004581	Methionine showed an even stronger retarding effect on MPO-induced LDL modification among the HOCl traps used (factor 103), while glycine was the least effective (factor 13,  Fig. 5).	transcription
53281	3	335067	7	NULL	NULL	0	NULL	glycine	NULL		retard	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1481_1_109_s_167	11004581	Methionine showed an even stronger retarding effect on MPO-induced LDL modification among the HOCl traps used (factor 103), while glycine was the least effective (factor 13,  Fig. 5).	transcription
53282	4	335067	7	NULL	NULL	0	NULL	statement 2	NULL	retarding effect of	is stronger than	NULL				statement 3	NULL	retarding effect of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1481_1_109_s_167	11004581	Methionine showed an even stronger retarding effect on MPO-induced LDL modification among the HOCl traps used (factor 103), while glycine was the least effective (factor 13,  Fig. 5).	transcription
53509	1	335070	5	NULL	NULL	0	NULL	glutamate	NULL		activates	NULL				NR1/NR2A receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53510	2	335070	5	NULL	NULL	0	NULL	glutamate	NULL		activates	NULL				NR1/NR2B receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53511	3	335070	5	NULL	NULL	0	NULL	glutamate	NULL		activates	NULL				NR1/NR2C receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53512	4	335070	5	NULL	NULL	0	NULL	glutamate	NULL		activates	NULL				NR1/NR2D receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53513	5	335070	5	NULL	NULL	0	NULL	glycine	NULL		activates	NULL				NR1/NR2A receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53514	6	335070	5	NULL	NULL	0	NULL	glycine	NULL		activates	NULL				NR1/NR2B receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53515	7	335070	5	NULL	NULL	0	NULL	glycine	NULL		activates	NULL				NR1/NR2C receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53516	8	335070	5	NULL	NULL	0	NULL	glycine	NULL		activates	NULL				NR1/NR2D receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53517	9	335070	5	NULL	NULL	0	NULL	3alpha5betaS	NULL		decreases	NULL				statement 1	NULL	efficacy of			NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53518	10	335070	5	NULL	NULL	0	NULL	3alpha5betaS	NULL		decreases	NULL				statement 2	NULL	efficacy of			NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53519	11	335070	5	NULL	NULL	0	NULL	3alpha5betaS	NULL		decreases	NULL				statement 3	NULL	efficacy of			NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53520	12	335070	5	NULL	NULL	0	NULL	3alpha5betaS	NULL		decreases	NULL				statement 4	NULL	efficacy of			NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53521	13	335070	5	NULL	NULL	0	NULL	3alpha5betaS	NULL		decreases	NULL				statement 5	NULL	efficacy of			NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53522	14	335070	5	NULL	NULL	0	NULL	3alpha5betaS	NULL		decreases	NULL				statement 6	NULL	efficacy of			NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53523	15	335070	5	NULL	NULL	0	NULL	3alpha5betaS	NULL		decreases	NULL				statement 7	NULL	efficacy of			NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53524	16	335070	5	NULL	NULL	0	NULL	3alpha5betaS	NULL		decreases	NULL				statement 8	NULL	efficacy of			NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53283	1	335070	7	NULL	NULL	0	NULL	glutamate	NULL		activate	NULL				NR1/NR2A receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53284	2	335070	7	NULL	NULL	0	NULL	glutamate	NULL		activate	NULL				NR1/NR2B receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53285	3	335070	7	NULL	NULL	0	NULL	glutamate 	NULL		activate	NULL				NR1/NR2C receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53286	4	335070	7	NULL	NULL	0	NULL	glutamate	NULL		activate	NULL				NR1/NR2D receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53287	5	335070	7	NULL	NULL	0	NULL	glycine	NULL		activate	NULL				NR1/NR2A receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53288	6	335070	7	NULL	NULL	0	NULL	glycine	NULL		activate	NULL				NR1/NR2B receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53289	7	335070	7	NULL	NULL	0	NULL	glycine	NULL		activate	NULL				NR1/NR2C receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53290	8	335070	7	NULL	NULL	0	NULL	glycine	NULL		activate	NULL				NR1/NR2D receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53291	9	335070	7	NULL	NULL	0	NULL	3alpha5betaS	NULL		decrease	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53292	10	335070	7	NULL	NULL	0	NULL	3alpha5betaS	NULL		decrease	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53293	11	335070	7	NULL	NULL	0	NULL	3alpha5betaS	NULL		decrease	NULL				statement 3	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53294	12	335070	7	NULL	NULL	0	NULL	3alpha5betaS	NULL		decrease	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53295	13	335070	7	NULL	NULL	0	NULL	3alpha5betaS	NULL		decrease	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53296	14	335070	7	NULL	NULL	0	NULL	3alpha5betaS	NULL		decrease	NULL				statement 6	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53297	15	335070	7	NULL	NULL	0	NULL	3alpha5betaS	NULL		decrease	NULL				statement 7	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53298	16	335070	7	NULL	NULL	0	NULL	3alpha5betaS	NULL		decrease	NULL				statement 8	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_4_901_s_135	11861317	As shown in  Figure 5, 3alpha5betaS decreases the efficacy with which glutamate and glycine activate NR1/NR2A ( Figure 5a,b), NR1/NR2B ( Figure 5c,d), NR1/NR2C ( Figure 5e,f), and NR1/NR2D ( Figure 5g,h) receptors.	transcription
53525	1	335071	5	NULL	NULL	0	NULL	5-HT1A receptor	NULL		affinity for	NULL	high	binding sites		8-OH-DPAT	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_137_3_345_s_7	12237254	5 The proportion of 5-HT1A receptor binding sites detected by [3]-MPPF that displayed high affinity for 8-OH-DPAT was significantly greater when the interacting G protein contained isoleucine rather than glycine at residue351.	transcription
53526	2	335071	5	NULL	NULL	0	NULL	interacting G protein	NULL		contains	NULL					NULL		isoleucine residue 351		NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_137_3_345_s_7	12237254	5 The proportion of 5-HT1A receptor binding sites detected by [3]-MPPF that displayed high affinity for 8-OH-DPAT was significantly greater when the interacting G protein contained isoleucine rather than glycine at residue351.	transcription
53527	3	335071	5	NULL	NULL	0	NULL	interacting G protein	NULL		contains	NULL					NULL		glycine residue351		NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_137_3_345_s_7	12237254	5 The proportion of 5-HT1A receptor binding sites detected by [3]-MPPF that displayed high affinity for 8-OH-DPAT was significantly greater when the interacting G protein contained isoleucine rather than glycine at residue351.	transcription
53299	1	335071	7	NULL	NULL	0	NULL	5-HT1A receptor	NULL		high affinity for	NULL		binding sites		8-OH-DPAT	NULL				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_137_3_345_s_7	12237254	5 The proportion of 5-HT1A receptor binding sites detected by [3]-MPPF that displayed high affinity for 8-OH-DPAT was significantly greater when the interacting G protein contained isoleucine rather than glycine at residue351.	transcription
53300	2	335071	7	NULL	NULL	0	NULL	interacting G protein	NULL		contains	NULL					NULL		isoleucine residue 351		NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_137_3_345_s_7	12237254	5 The proportion of 5-HT1A receptor binding sites detected by [3]-MPPF that displayed high affinity for 8-OH-DPAT was significantly greater when the interacting G protein contained isoleucine rather than glycine at residue351.	transcription
53301	3	335071	7	NULL	NULL	0	NULL	interacting G protein	NULL		contains	NULL					NULL		glycine residue 351		NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_137_3_345_s_7	12237254	5 The proportion of 5-HT1A receptor binding sites detected by [3]-MPPF that displayed high affinity for 8-OH-DPAT was significantly greater when the interacting G protein contained isoleucine rather than glycine at residue351.	transcription
53305	4	335071	7	NULL	NULL	0	NULL	statement 2	NULL	affinity of	is higher than	NULL				statement 3	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_137_3_345_s_7	12237254	5 The proportion of 5-HT1A receptor binding sites detected by [3]-MPPF that displayed high affinity for 8-OH-DPAT was significantly greater when the interacting G protein contained isoleucine rather than glycine at residue351.	transcription
53528	1	335072	5	NULL	NULL	0	NULL	glycine	NULL	substitution of	affects	NULL	may				NULL	secondary structure of	region following the helix 5		NULL		0	NULL	NULL	NULL	gw60_chembiol_7_9_709_s_114	10980451	Their substitution for glycine may affect the secondary structure of the region following the helix  5, not only because of an increased flexibility, but also because of the loss of hydrogen bonds between the side chains of S149 and Ser164, and nearby residues.	transcription
53529	2	335072	5	NULL	NULL	0	NULL	flexibility	NULL	increased	leads to	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_chembiol_7_9_709_s_114	10980451	Their substitution for glycine may affect the secondary structure of the region following the helix  5, not only because of an increased flexibility, but also because of the loss of hydrogen bonds between the side chains of S149 and Ser164, and nearby residues.	transcription
53530	3	335072	5	NULL	NULL	0	NULL	hydrogen bonds	NULL		is lost between	NULL					NULL	side chains of	S149;;Ser164		NULL		0	NULL	NULL	NULL	gw60_chembiol_7_9_709_s_114	10980451	Their substitution for glycine may affect the secondary structure of the region following the helix  5, not only because of an increased flexibility, but also because of the loss of hydrogen bonds between the side chains of S149 and Ser164, and nearby residues.	transcription
53531	4	335072	5	NULL	NULL	0	NULL	statement 3	NULL		leads to	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_chembiol_7_9_709_s_114	10980451	Their substitution for glycine may affect the secondary structure of the region following the helix  5, not only because of an increased flexibility, but also because of the loss of hydrogen bonds between the side chains of S149 and Ser164, and nearby residues.	transcription
53306	1	335072	7	NULL	NULL	0	NULL	glycine	NULL	 substitution for	affect	NULL					NULL	secondary structure of 	region following helix 5		NULL		0	NULL	NULL	NULL	gw60_chembiol_7_9_709_s_114	10980451	Their substitution for glycine may affect the secondary structure of the region following the helix  5, not only because of an increased flexibility, but also because of the loss of hydrogen bonds between the side chains of S149 and Ser164, and nearby residues.	transcription
53307	2	335072	7	NULL	NULL	0	NULL	statement 1	NULL		because of	NULL				increased flexibility	NULL				NULL		0	NULL	NULL	NULL	gw60_chembiol_7_9_709_s_114	10980451	Their substitution for glycine may affect the secondary structure of the region following the helix  5, not only because of an increased flexibility, but also because of the loss of hydrogen bonds between the side chains of S149 and Ser164, and nearby residues.	transcription
53308	3	335072	7	NULL	NULL	0	NULL	statement 1	NULL		because of	NULL				hydrogen bonds	NULL	loss of	between side chains of S149 and Ser164		NULL		NULL	NULL	NULL	NULL	gw60_chembiol_7_9_709_s_114	10980451	Their substitution for glycine may affect the secondary structure of the region following the helix  5, not only because of an increased flexibility, but also because of the loss of hydrogen bonds between the side chains of S149 and Ser164, and nearby residues.	transcription
53532	1	335080	5	NULL	NULL	0	NULL	ivermectin	NULL		induce	NULL				GlyR	NULL	direct;;activation of;;mutant	R271Q		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_16_12556_s_174	11278873	Although 0.03 muM ivermectin induced little direct activation of the R271Q mutant GlyR, it potentiated the magnitude of currents activated by a 7 mM (EC50) concentration of glycine (Fig.  5 A).	transcription
53309	1	335080	7	NULL	NULL	0	NULL	ivermectin	NULL		induce	NULL				GlyR	NULL	direct activation of ;;mutant	R271Q 		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_16_12556_s_174	11278873	Although 0.03 muM ivermectin induced little direct activation of the R271Q mutant GlyR, it potentiated the magnitude of currents activated by a 7 mM (EC50) concentration of glycine (Fig.  5 A).	transcription
53533	1	335082	5	NULL	NULL	0	NULL	EGF-R peptide	NULL	aromatic residues of	is mutated to	NULL				EGF-R peptide	NULL		glycine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_48_30429_s_160	9374534	In accordance with these observations, a mutated EGF-R peptide in which all aromatic residues were changed to glycine failed to interact with the caveolin 1 scaffolding domain (Fig.  5 A).	transcription
53534	2	335082	5	NULL	NULL	0	NULL	statement 1	NULL		does not interact with	NULL				caveolin 1	NULL		scaffolding domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_48_30429_s_160	9374534	In accordance with these observations, a mutated EGF-R peptide in which all aromatic residues were changed to glycine failed to interact with the caveolin 1 scaffolding domain (Fig.  5 A).	transcription
53310	1	335082	7	NULL	NULL	0	NULL	EGF-R peptide	NULL		changed to	NULL		aromatic residues 		EGF-R peptide	NULL	mutant	glycine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_48_30429_s_160	9374534	In accordance with these observations, a mutated EGF-R peptide in which all aromatic residues were changed to glycine failed to interact with the caveolin 1 scaffolding domain (Fig.  5 A).	transcription
53311	2	335082	7	NULL	NULL	0	NULL	statement 1	NULL		does not interact with	NULL				caveolin 1 	NULL		 scaffolding domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_48_30429_s_160	9374534	In accordance with these observations, a mutated EGF-R peptide in which all aromatic residues were changed to glycine failed to interact with the caveolin 1 scaffolding domain (Fig.  5 A).	transcription
53535	1	335084	5	NULL	NULL	0	NULL	polyamine	NULL	stimulation of	is independent of	NULL				glycine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_40_24971_s_128	9312102	Because glycine-independent polyamine stimulation may result from the relief of the tonic inhibition of the NMDA receptor by protons ( 39), the proton inhibition of the Glu-201 mutant receptors was investigated (Fig.  5,  A and  B).	transcription
53536	2	335084	5	NULL	NULL	0	NULL	protons	NULL		inhibit	NULL				NMDA receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_40_24971_s_128	9312102	Because glycine-independent polyamine stimulation may result from the relief of the tonic inhibition of the NMDA receptor by protons ( 39), the proton inhibition of the Glu-201 mutant receptors was investigated (Fig.  5,  A and  B).	transcription
53537	3	335084	5	NULL	NULL	0	NULL	statement 2	NULL	relief of	results in	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_40_24971_s_128	9312102	Because glycine-independent polyamine stimulation may result from the relief of the tonic inhibition of the NMDA receptor by protons ( 39), the proton inhibition of the Glu-201 mutant receptors was investigated (Fig.  5,  A and  B).	transcription
53312	1	335084	7	NULL	NULL	0	NULL	protons	NULL		inhibit	NULL				NMDA receptor	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_40_24971_s_128	9312102	Because glycine-independent polyamine stimulation may result from the relief of the tonic inhibition of the NMDA receptor by protons ( 39), the proton inhibition of the Glu-201 mutant receptors was investigated (Fig.  5,  A and  B).	transcription
53313	2	335084	7	NULL	NULL	0	NULL	statement 1	NULL		is a type of	NULL				tonic inhibition	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_40_24971_s_128	9312102	Because glycine-independent polyamine stimulation may result from the relief of the tonic inhibition of the NMDA receptor by protons ( 39), the proton inhibition of the Glu-201 mutant receptors was investigated (Fig.  5,  A and  B).	transcription
53314	3	335084	7	NULL	NULL	0	NULL	polyamine	NULL	stimulation of	independent of	NULL				glycine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_40_24971_s_128	9312102	Because glycine-independent polyamine stimulation may result from the relief of the tonic inhibition of the NMDA receptor by protons ( 39), the proton inhibition of the Glu-201 mutant receptors was investigated (Fig.  5,  A and  B).	transcription
53315	4	335084	7	NULL	NULL	0	NULL	statement 3	NULL		result from	NULL	may			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_40_24971_s_128	9312102	Because glycine-independent polyamine stimulation may result from the relief of the tonic inhibition of the NMDA receptor by protons ( 39), the proton inhibition of the Glu-201 mutant receptors was investigated (Fig.  5,  A and  B).	transcription
53316	5	335084	7	NULL	NULL	0	NULL	protons	NULL		inhibit	NULL				receptors	NULL	mutant	Glu-201		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_40_24971_s_128	9312102	Because glycine-independent polyamine stimulation may result from the relief of the tonic inhibition of the NMDA receptor by protons ( 39), the proton inhibition of the Glu-201 mutant receptors was investigated (Fig.  5,  A and  B).	transcription
53538	1	335085	5	NULL	NULL	0	NULL	glutamate	NULL		stimulates	NULL				NMDA receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_44_34252_s_238	10950953	Subsequent addition of 100 muML-glutamate and 10 muM glycine (stimulating both NMDA receptors and mGluRs)  reduced [Ca2+] i (Fig.  4 b;  n = 5).	transcription
53539	2	335085	5	NULL	NULL	0	NULL	glutamate	NULL		stimulates	NULL				mGluRs	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_44_34252_s_238	10950953	Subsequent addition of 100 muML-glutamate and 10 muM glycine (stimulating both NMDA receptors and mGluRs)  reduced [Ca2+] i (Fig.  4 b;  n = 5).	transcription
53540	3	335085	5	NULL	NULL	0	NULL	glycine	NULL		stimulates	NULL				NMDA receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_44_34252_s_238	10950953	Subsequent addition of 100 muML-glutamate and 10 muM glycine (stimulating both NMDA receptors and mGluRs)  reduced [Ca2+] i (Fig.  4 b;  n = 5).	transcription
53541	4	335085	5	NULL	NULL	0	NULL	glycine	NULL		stimulates	NULL				mGluRs	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_44_34252_s_238	10950953	Subsequent addition of 100 muML-glutamate and 10 muM glycine (stimulating both NMDA receptors and mGluRs)  reduced [Ca2+] i (Fig.  4 b;  n = 5).	transcription
53542	5	335085	5	NULL	NULL	0	NULL	statement 1	NULL		occurs along with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_44_34252_s_238	10950953	Subsequent addition of 100 muML-glutamate and 10 muM glycine (stimulating both NMDA receptors and mGluRs)  reduced [Ca2+] i (Fig.  4 b;  n = 5).	transcription
53543	6	335085	5	NULL	NULL	0	NULL	statement 5	NULL		reduces	NULL				[Ca2+] i	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_44_34252_s_238	10950953	Subsequent addition of 100 muML-glutamate and 10 muM glycine (stimulating both NMDA receptors and mGluRs)  reduced [Ca2+] i (Fig.  4 b;  n = 5).	transcription
53544	7	335085	5	NULL	NULL	0	NULL	statement 3	NULL		occurs along with	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_44_34252_s_238	10950953	Subsequent addition of 100 muML-glutamate and 10 muM glycine (stimulating both NMDA receptors and mGluRs)  reduced [Ca2+] i (Fig.  4 b;  n = 5).	transcription
53545	8	335085	5	NULL	NULL	0	NULL	statement 7	NULL		reduces	NULL				[Ca2+] i	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_44_34252_s_238	10950953	Subsequent addition of 100 muML-glutamate and 10 muM glycine (stimulating both NMDA receptors and mGluRs)  reduced [Ca2+] i (Fig.  4 b;  n = 5).	transcription
53317	1	335085	7	NULL	NULL	0	NULL	NMDA receptor	NULL	stimulation of	reduce	NULL				Ca2+	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_44_34252_s_238	10950953	Subsequent addition of 100 muML-glutamate and 10 muM glycine (stimulating both NMDA receptors and mGluRs)  reduced [Ca2+] i (Fig.  4 b;  n = 5).	transcription
53318	2	335085	7	NULL	NULL	0	NULL	mGluRs	NULL	stimulation of	reduce	NULL				Ca2+	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_44_34252_s_238	10950953	Subsequent addition of 100 muML-glutamate and 10 muM glycine (stimulating both NMDA receptors and mGluRs)  reduced [Ca2+] i (Fig.  4 b;  n = 5).	transcription
53319	3	335085	7	NULL	NULL	0	NULL	statement 1	NULL		occur along with	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_44_34252_s_238	10950953	Subsequent addition of 100 muML-glutamate and 10 muM glycine (stimulating both NMDA receptors and mGluRs)  reduced [Ca2+] i (Fig.  4 b;  n = 5).	transcription
53546	1	335086	5	NULL	NULL	0	NULL	OATP2	NULL	human	transports	NULL				cholyl taurine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_30_23161_s_278	10779507	In contrast to human OATP2, which transports cholyl taurine and whose 17beta-glucuronosyl estradiol transport was inhibited by cholate ( 5), OATP8 did neither transport cholyl taurine nor cholate nor cholyl glycine.	transcription
53547	2	335086	5	NULL	NULL	0	NULL	OATP2	NULL	human	transports	NULL				17beta-glucuronosyl estradiol	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_30_23161_s_278	10779507	In contrast to human OATP2, which transports cholyl taurine and whose 17beta-glucuronosyl estradiol transport was inhibited by cholate ( 5), OATP8 did neither transport cholyl taurine nor cholate nor cholyl glycine.	transcription
53548	3	335086	5	NULL	NULL	0	NULL	cholate	NULL		inhibits	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_30_23161_s_278	10779507	In contrast to human OATP2, which transports cholyl taurine and whose 17beta-glucuronosyl estradiol transport was inhibited by cholate ( 5), OATP8 did neither transport cholyl taurine nor cholate nor cholyl glycine.	transcription
53549	4	335086	5	NULL	NULL	0	NULL	OATP8	NULL		does not transport	NULL				cholyl taurine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_30_23161_s_278	10779507	In contrast to human OATP2, which transports cholyl taurine and whose 17beta-glucuronosyl estradiol transport was inhibited by cholate ( 5), OATP8 did neither transport cholyl taurine nor cholate nor cholyl glycine.	transcription
53550	5	335086	5	NULL	NULL	0	NULL	OATP8	NULL		does not transport	NULL				cholate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_30_23161_s_278	10779507	In contrast to human OATP2, which transports cholyl taurine and whose 17beta-glucuronosyl estradiol transport was inhibited by cholate ( 5), OATP8 did neither transport cholyl taurine nor cholate nor cholyl glycine.	transcription
53551	6	335086	5	NULL	NULL	0	NULL	OATP8	NULL		does not transport	NULL				cholyl glycine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_30_23161_s_278	10779507	In contrast to human OATP2, which transports cholyl taurine and whose 17beta-glucuronosyl estradiol transport was inhibited by cholate ( 5), OATP8 did neither transport cholyl taurine nor cholate nor cholyl glycine.	transcription
53320	1	335086	7	NULL	NULL	0	NULL	OATP2	NULL	human	transports	NULL				cholyl taurine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_30_23161_s_278	10779507	In contrast to human OATP2, which transports cholyl taurine and whose 17beta-glucuronosyl estradiol transport was inhibited by cholate ( 5), OATP8 did neither transport cholyl taurine nor cholate nor cholyl glycine.	transcription
53321	2	335086	7	NULL	NULL	0	NULL	cholate	NULL		inhibit	NULL				17beta-glucuronosyl estradiol	NULL	transport of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_30_23161_s_278	10779507	In contrast to human OATP2, which transports cholyl taurine and whose 17beta-glucuronosyl estradiol transport was inhibited by cholate ( 5), OATP8 did neither transport cholyl taurine nor cholate nor cholyl glycine.	transcription
53322	3	335086	7	NULL	NULL	0	NULL	OATP8	NULL		does not transport	NULL				cholyl taurine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_30_23161_s_278	10779507	In contrast to human OATP2, which transports cholyl taurine and whose 17beta-glucuronosyl estradiol transport was inhibited by cholate ( 5), OATP8 did neither transport cholyl taurine nor cholate nor cholyl glycine.	transcription
53323	4	335086	7	NULL	NULL	0	NULL	OATP8	NULL		does not transport	NULL				cholate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_30_23161_s_278	10779507	In contrast to human OATP2, which transports cholyl taurine and whose 17beta-glucuronosyl estradiol transport was inhibited by cholate ( 5), OATP8 did neither transport cholyl taurine nor cholate nor cholyl glycine.	transcription
53324	5	335086	7	NULL	NULL	0	NULL	OATP8	NULL		does not transport	NULL				cholyl glycine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_30_23161_s_278	10779507	In contrast to human OATP2, which transports cholyl taurine and whose 17beta-glucuronosyl estradiol transport was inhibited by cholate ( 5), OATP8 did neither transport cholyl taurine nor cholate nor cholyl glycine.	transcription
53552	1	335088	5	NULL	NULL	0	NULL	NMDA receptors	NULL		is a type of	NULL				heteromers	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_1_276_s_11	12414797	NMDA receptors are heteromers containing NR1 subunits, which bind the co-agonist glycine ( 2,  3), and NR2 subunits, which bind the agonist glutamate ( 4,  5).	transcription
53553	2	335088	5	NULL	NULL	0	NULL	NMDA receptors	NULL		contains	NULL					NULL		NR1 subunits		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_1_276_s_11	12414797	NMDA receptors are heteromers containing NR1 subunits, which bind the co-agonist glycine ( 2,  3), and NR2 subunits, which bind the agonist glutamate ( 4,  5).	transcription
53554	3	335088	5	NULL	NULL	0	NULL	NMDA receptors	NULL		bind	NULL		NR1 subunits		glycine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_1_276_s_11	12414797	NMDA receptors are heteromers containing NR1 subunits, which bind the co-agonist glycine ( 2,  3), and NR2 subunits, which bind the agonist glutamate ( 4,  5).	transcription
53555	4	335088	5	NULL	NULL	0	NULL	glycine	NULL		is a type of	NULL				co-agonist	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_1_276_s_11	12414797	NMDA receptors are heteromers containing NR1 subunits, which bind the co-agonist glycine ( 2,  3), and NR2 subunits, which bind the agonist glutamate ( 4,  5).	transcription
53556	5	335088	5	NULL	NULL	0	NULL	NMDA receptors	NULL		contains	NULL					NULL		NR2 subunits		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_1_276_s_11	12414797	NMDA receptors are heteromers containing NR1 subunits, which bind the co-agonist glycine ( 2,  3), and NR2 subunits, which bind the agonist glutamate ( 4,  5).	transcription
53557	6	335088	5	NULL	NULL	0	NULL	NMDA receptors	NULL		bind	NULL		NR2 subunits		glutamate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_1_276_s_11	12414797	NMDA receptors are heteromers containing NR1 subunits, which bind the co-agonist glycine ( 2,  3), and NR2 subunits, which bind the agonist glutamate ( 4,  5).	transcription
53558	7	335088	5	NULL	NULL	0	NULL	glutamate	NULL		is a type of	NULL				agonist	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_1_276_s_11	12414797	NMDA receptors are heteromers containing NR1 subunits, which bind the co-agonist glycine ( 2,  3), and NR2 subunits, which bind the agonist glutamate ( 4,  5).	transcription
53325	1	335088	7	NULL	NULL	0	NULL	NMDA receptors	NULL		contains	NULL					NULL		NR1 subunits		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_1_276_s_11	12414797	NMDA receptors are heteromers containing NR1 subunits, which bind the co-agonist glycine ( 2,  3), and NR2 subunits, which bind the agonist glutamate ( 4,  5).	transcription
53326	2	335088	7	NULL	NULL	0	NULL	statement 1	NULL		bind	NULL				glycine	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_1_276_s_11	12414797	NMDA receptors are heteromers containing NR1 subunits, which bind the co-agonist glycine ( 2,  3), and NR2 subunits, which bind the agonist glutamate ( 4,  5).	transcription
53327	3	335088	7	NULL	NULL	0	NULL	NMDA receptors	NULL		is a type of	NULL				heteromer	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_1_276_s_11	12414797	NMDA receptors are heteromers containing NR1 subunits, which bind the co-agonist glycine ( 2,  3), and NR2 subunits, which bind the agonist glutamate ( 4,  5).	transcription
53328	4	335088	7	NULL	NULL	0	NULL	NMDA receptors	NULL		contain	NULL					NULL		NR2 subunits		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_1_276_s_11	12414797	NMDA receptors are heteromers containing NR1 subunits, which bind the co-agonist glycine ( 2,  3), and NR2 subunits, which bind the agonist glutamate ( 4,  5).	transcription
53329	5	335088	7	NULL	NULL	0	NULL	statement 4	NULL		bind	NULL				glutamate	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_1_276_s_11	12414797	NMDA receptors are heteromers containing NR1 subunits, which bind the co-agonist glycine ( 2,  3), and NR2 subunits, which bind the agonist glutamate ( 4,  5).	transcription
53330	6	335088	7	NULL	NULL	0	NULL	glycine	NULL		is a type of	NULL				co-agonist	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_1_276_s_11	12414797	NMDA receptors are heteromers containing NR1 subunits, which bind the co-agonist glycine ( 2,  3), and NR2 subunits, which bind the agonist glutamate ( 4,  5).	transcription
53331	7	335088	7	NULL	NULL	0	NULL	 glutamate	NULL		is a type of	NULL				agonist	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_1_276_s_11	12414797	NMDA receptors are heteromers containing NR1 subunits, which bind the co-agonist glycine ( 2,  3), and NR2 subunits, which bind the agonist glutamate ( 4,  5).	transcription
53559	1	335092	5	NULL	NULL	0	NULL	GABAA receptors		mutation of	affects					anesthetic 		action of;;volatile			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_14_8248_s_202	9525931	Because mutations of GABAA and glycine receptors that affect volatile anesthetic actions also affect alcohol (but not barbiturate) actions ( 5), we asked if mutation of Gly-819 would change ethanol and pentobarbital inhibition of GluR6.	transcription
54027	2	335092	5	NULL	NULL	0	NULL	GABAA receptors		mutation of	affects					alcohol		action of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8248_s_202	9525931	Because mutations of GABAA and glycine receptors that affect volatile anesthetic actions also affect alcohol (but not barbiturate) actions ( 5), we asked if mutation of Gly-819 would change ethanol and pentobarbital inhibition of GluR6.	transcription
54028	3	335092	5	NULL	NULL	0	NULL	GABAA receptors		mutation of	does not affect					barbiturate		action of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8248_s_202	9525931	Because mutations of GABAA and glycine receptors that affect volatile anesthetic actions also affect alcohol (but not barbiturate) actions ( 5), we asked if mutation of Gly-819 would change ethanol and pentobarbital inhibition of GluR6.	transcription
54029	4	335092	5	NULL	NULL	0	NULL	glycine receptors		mutation of	affects					anesthetic		action of;;volatile			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8248_s_202	9525931	Because mutations of GABAA and glycine receptors that affect volatile anesthetic actions also affect alcohol (but not barbiturate) actions ( 5), we asked if mutation of Gly-819 would change ethanol and pentobarbital inhibition of GluR6.	transcription
54030	5	335092	5	NULL	NULL	0	NULL	glycine receptors		mutation of	affects					alcohol		action of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8248_s_202	9525931	Because mutations of GABAA and glycine receptors that affect volatile anesthetic actions also affect alcohol (but not barbiturate) actions ( 5), we asked if mutation of Gly-819 would change ethanol and pentobarbital inhibition of GluR6.	transcription
54031	6	335092	5	NULL	NULL	0	NULL	glycine receptors			does not affect					barbiturate		action of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8248_s_202	9525931	Because mutations of GABAA and glycine receptors that affect volatile anesthetic actions also affect alcohol (but not barbiturate) actions ( 5), we asked if mutation of Gly-819 would change ethanol and pentobarbital inhibition of GluR6.	transcription
53332	1	335092	7	NULL	NULL	0	NULL	GABAA receptors		mutation of	affect					 volatile anesthetic 		action of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_14_8248_s_202	9525931	Because mutations of GABAA and glycine receptors that affect volatile anesthetic actions also affect alcohol (but not barbiturate) actions ( 5), we asked if mutation of Gly-819 would change ethanol and pentobarbital inhibition of GluR6.	transcription
53333	2	335092	7	NULL	NULL	0	NULL	GABAA receptors		mutation of	affect					alcohol		action of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_14_8248_s_202	9525931	Because mutations of GABAA and glycine receptors that affect volatile anesthetic actions also affect alcohol (but not barbiturate) actions ( 5), we asked if mutation of Gly-819 would change ethanol and pentobarbital inhibition of GluR6.	transcription
53334	3	335092	7	NULL	NULL	0	NULL	GABAA receptors		mutation of	does not affect					barbiturate		action of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_14_8248_s_202	9525931	Because mutations of GABAA and glycine receptors that affect volatile anesthetic actions also affect alcohol (but not barbiturate) actions ( 5), we asked if mutation of Gly-819 would change ethanol and pentobarbital inhibition of GluR6.	transcription
53335	4	335092	7	NULL	NULL	0	NULL	glycine receptors		mutation of	affect					volatile anesthetic 		action of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_14_8248_s_202	9525931	Because mutations of GABAA and glycine receptors that affect volatile anesthetic actions also affect alcohol (but not barbiturate) actions ( 5), we asked if mutation of Gly-819 would change ethanol and pentobarbital inhibition of GluR6.	transcription
53336	5	335092	7	NULL	NULL	0	NULL	glycine receptors		mutation of	affect					alchol		action of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_14_8248_s_202	9525931	Because mutations of GABAA and glycine receptors that affect volatile anesthetic actions also affect alcohol (but not barbiturate) actions ( 5), we asked if mutation of Gly-819 would change ethanol and pentobarbital inhibition of GluR6.	transcription
53337	6	335092	7	NULL	NULL	0	NULL	glycine receptors		mutation of	does not affect					barbiturate		action of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_14_8248_s_202	9525931	Because mutations of GABAA and glycine receptors that affect volatile anesthetic actions also affect alcohol (but not barbiturate) actions ( 5), we asked if mutation of Gly-819 would change ethanol and pentobarbital inhibition of GluR6.	transcription
53560	1	335093	5	NULL	NULL	0	NULL	NMDA receptors	NULL		permeable to	NULL	highly			Ca2+	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_32_19933_s_11	9685327	NMDA receptors are highly permeable to Ca2+ ( 3), they are regulated by a voltage-dependent Mg2+ block ( 4), and simultaneous binding of both glutamate and the co-agonist glycine is required for efficient activation of NMDA receptors ( 5,  6).	transcription
53561	2	335093	5	NULL	NULL	0	NULL	Mg2+	NULL	blocking of	is dependent on	NULL				voltage	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_32_19933_s_11	9685327	NMDA receptors are highly permeable to Ca2+ ( 3), they are regulated by a voltage-dependent Mg2+ block ( 4), and simultaneous binding of both glutamate and the co-agonist glycine is required for efficient activation of NMDA receptors ( 5,  6).	transcription
53562	3	335093	5	NULL	NULL	0	NULL	statement 2	NULL		regulates	NULL				NMDA receptors	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_32_19933_s_11	9685327	NMDA receptors are highly permeable to Ca2+ ( 3), they are regulated by a voltage-dependent Mg2+ block ( 4), and simultaneous binding of both glutamate and the co-agonist glycine is required for efficient activation of NMDA receptors ( 5,  6).	transcription
53563	4	335093	5	NULL	NULL	0	NULL	glutamate	NULL	binding of	occurs simultaneously with	NULL				glycine	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_32_19933_s_11	9685327	NMDA receptors are highly permeable to Ca2+ ( 3), they are regulated by a voltage-dependent Mg2+ block ( 4), and simultaneous binding of both glutamate and the co-agonist glycine is required for efficient activation of NMDA receptors ( 5,  6).	transcription
53564	5	335093	5	NULL	NULL	0	NULL	statement 4	NULL		is required for	NULL				NMDA receptors	NULL	efficient activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_32_19933_s_11	9685327	NMDA receptors are highly permeable to Ca2+ ( 3), they are regulated by a voltage-dependent Mg2+ block ( 4), and simultaneous binding of both glutamate and the co-agonist glycine is required for efficient activation of NMDA receptors ( 5,  6).	transcription
53565	6	335093	5	NULL	NULL	0	NULL	glycine	NULL		is a type of	NULL				co-agonist	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_32_19933_s_11	9685327	NMDA receptors are highly permeable to Ca2+ ( 3), they are regulated by a voltage-dependent Mg2+ block ( 4), and simultaneous binding of both glutamate and the co-agonist glycine is required for efficient activation of NMDA receptors ( 5,  6).	transcription
53338	1	335093	7	NULL	NULL	0	NULL	NMDA receptors	NULL		permeable to	NULL	highly			Ca2+	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_32_19933_s_11	9685327	NMDA receptors are highly permeable to Ca2+ ( 3), they are regulated by a voltage-dependent Mg2+ block ( 4), and simultaneous binding of both glutamate and the co-agonist glycine is required for efficient activation of NMDA receptors ( 5,  6).	transcription
53339	2	335093	7	NULL	NULL	0	NULL	Mg2+	NULL	blocking of	depends on	NULL				voltage	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_32_19933_s_11	9685327	NMDA receptors are highly permeable to Ca2+ ( 3), they are regulated by a voltage-dependent Mg2+ block ( 4), and simultaneous binding of both glutamate and the co-agonist glycine is required for efficient activation of NMDA receptors ( 5,  6).	transcription
53340	3	335093	7	NULL	NULL	0	NULL	NMDA receptors	NULL		regulated by	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_32_19933_s_11	9685327	NMDA receptors are highly permeable to Ca2+ ( 3), they are regulated by a voltage-dependent Mg2+ block ( 4), and simultaneous binding of both glutamate and the co-agonist glycine is required for efficient activation of NMDA receptors ( 5,  6).	transcription
53341	4	335093	7	NULL	NULL	0	NULL	glutamate	NULL	binding of	is required for	NULL				NMDA receptors	NULL	efficient activation of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_32_19933_s_11	9685327	NMDA receptors are highly permeable to Ca2+ ( 3), they are regulated by a voltage-dependent Mg2+ block ( 4), and simultaneous binding of both glutamate and the co-agonist glycine is required for efficient activation of NMDA receptors ( 5,  6).	transcription
53342	5	335093	7	NULL	NULL	0	NULL	glycine	NULL	binding of	is required for	NULL				NMDA receptors	NULL	efficient activation of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_32_19933_s_11	9685327	NMDA receptors are highly permeable to Ca2+ ( 3), they are regulated by a voltage-dependent Mg2+ block ( 4), and simultaneous binding of both glutamate and the co-agonist glycine is required for efficient activation of NMDA receptors ( 5,  6).	transcription
53343	6	335093	7	NULL	NULL	0	NULL	statement 4	NULL		occur simultaneously with	NULL				statement 5	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_32_19933_s_11	9685327	NMDA receptors are highly permeable to Ca2+ ( 3), they are regulated by a voltage-dependent Mg2+ block ( 4), and simultaneous binding of both glutamate and the co-agonist glycine is required for efficient activation of NMDA receptors ( 5,  6).	transcription
53344	2	335095	7	NULL	NULL	0	NULL	FSS	NULL	Mg2+-free	stimulate	NULL				NMDA receptors	NULL				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_18_10_3725_s_57	9570803	For stimulation of NMDA receptors, 100 muM NMDA in Mg2+-free FSS containing 5 muM glycine was perfused through the chamber for 80 sec, followed by FSS for 3 min.	transcription
53345	1	335095	7	NULL	NULL	0	NULL	FSS	NULL		contains	NULL				glycine	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_18_10_3725_s_57	9570803	For stimulation of NMDA receptors, 100 muM NMDA in Mg2+-free FSS containing 5 muM glycine was perfused through the chamber for 80 sec, followed by FSS for 3 min.	transcription
53566	1	335096	5	NULL	NULL	0	NULL	bicuculline	NULL		block	NULL	selectively			GABAA receptor-mediated responses	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_21_8482_s_195	11606637	These data show that 5 muM bicuculline can selectively block the majority of GABAA receptor-mediated responses, without having a large effect on the glycine receptor-mediated responses.	transcription
53567	2	335096	5	NULL	NULL	0	NULL	bicuculline	NULL		effect	NULL	may			glycine receptor-mediated responses	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_21_8482_s_195	11606637	These data show that 5 muM bicuculline can selectively block the majority of GABAA receptor-mediated responses, without having a large effect on the glycine receptor-mediated responses.	transcription
53346	1	335096	7	NULL	NULL	0	NULL	bicuculline	NULL		block	NULL	selectively			GABAA receptor-mediated responses	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_21_8482_s_195	11606637	These data show that 5 muM bicuculline can selectively block the majority of GABAA receptor-mediated responses, without having a large effect on the glycine receptor-mediated responses.	transcription
53347	2	335096	7	NULL	NULL	0	NULL	bicuculline	NULL		does not effect	NULL				glycine receptor-mediated responses	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_21_8482_s_195	11606637	These data show that 5 muM bicuculline can selectively block the majority of GABAA receptor-mediated responses, without having a large effect on the glycine receptor-mediated responses.	transcription
53568	1	335098	5	NULL	NULL	0	NULL	PMA	NULL		enhance	NULL				Ip	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_12_4452_s_173	10844014	In recordings made with EGTA, applications of PMA enhanced  Ip but had little effect on  Iss evoked by applying relatively intermediate concentrations of agonist and coagonist (50 muM NMDA and 0.5 muM glycine; Fig.  5 A).	transcription
53569	2	335098	5	NULL	NULL	0	NULL	PMA	NULL		effect	NULL	little			Iss	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_12_4452_s_173	10844014	In recordings made with EGTA, applications of PMA enhanced  Ip but had little effect on  Iss evoked by applying relatively intermediate concentrations of agonist and coagonist (50 muM NMDA and 0.5 muM glycine; Fig.  5 A).	transcription
53348	1	335098	7	NULL	NULL	0	NULL	PMA	NULL		enhance	NULL				Ip	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_12_4452_s_173	10844014	In recordings made with EGTA, applications of PMA enhanced  Ip but had little effect on  Iss evoked by applying relatively intermediate concentrations of agonist and coagonist (50 muM NMDA and 0.5 muM glycine; Fig.  5 A).	transcription
53349	2	335098	7	NULL	NULL	0	NULL	PMA	NULL		effect	NULL	little			Iss	NULL				NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_12_4452_s_173	10844014	In recordings made with EGTA, applications of PMA enhanced  Ip but had little effect on  Iss evoked by applying relatively intermediate concentrations of agonist and coagonist (50 muM NMDA and 0.5 muM glycine; Fig.  5 A).	transcription
53570	1	335101	5	NULL	NULL	0	NULL	Kupffer cells	NULL	activation of	is induced by	NULL				CsA	NULL				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_299_3_858_s_10	11714869	Importantly, dietary glycine (5%) largely blocked chronic CsA-induced activation of Kupffer cells, blunted production of PGE2, prevented the hypermetabolic state, and minimized tissue hypoxia.	transcription
53571	2	335101	5	NULL	NULL	0	NULL	glycine	NULL	dietary	block	NULL	largely			statement 1	NULL				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_299_3_858_s_10	11714869	Importantly, dietary glycine (5%) largely blocked chronic CsA-induced activation of Kupffer cells, blunted production of PGE2, prevented the hypermetabolic state, and minimized tissue hypoxia.	transcription
53573	3	335101	5	NULL	NULL	0	NULL	glycine	NULL	dietary	blunted	NULL				PGE2	NULL	production of			NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_299_3_858_s_10	11714869	Importantly, dietary glycine (5%) largely blocked chronic CsA-induced activation of Kupffer cells, blunted production of PGE2, prevented the hypermetabolic state, and minimized tissue hypoxia.	transcription
53574	4	335101	5	NULL	NULL	0	NULL	glycine	NULL	dietary	prevents	NULL				hypermetabolic state	NULL				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_299_3_858_s_10	11714869	Importantly, dietary glycine (5%) largely blocked chronic CsA-induced activation of Kupffer cells, blunted production of PGE2, prevented the hypermetabolic state, and minimized tissue hypoxia.	transcription
53575	5	335101	5	NULL	NULL	0	NULL	glycine	NULL	dietary	minimize	NULL				tissue hypoxia	NULL				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_299_3_858_s_10	11714869	Importantly, dietary glycine (5%) largely blocked chronic CsA-induced activation of Kupffer cells, blunted production of PGE2, prevented the hypermetabolic state, and minimized tissue hypoxia.	transcription
54018	1	335101	7	NULL	NULL	0	NULL	chronic CsA			induce					Kupffer cells		activation of			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_299_3_858_s_10	11714869	Importantly, dietary glycine (5%) largely blocked chronic CsA-induced activation of Kupffer cells, blunted production of PGE2, prevented the hypermetabolic state, and minimized tissue hypoxia.	transcription
54019	2	335101	7	NULL	NULL	0	NULL	dietary glycine			blocks		largely			statement 1					NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_299_3_858_s_10	11714869	Importantly, dietary glycine (5%) largely blocked chronic CsA-induced activation of Kupffer cells, blunted production of PGE2, prevented the hypermetabolic state, and minimized tissue hypoxia.	transcription
54020	3	335101	7	NULL	NULL	0	NULL	dietary glycine			blunt					PGE2		production of			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_299_3_858_s_10	11714869	Importantly, dietary glycine (5%) largely blocked chronic CsA-induced activation of Kupffer cells, blunted production of PGE2, prevented the hypermetabolic state, and minimized tissue hypoxia.	transcription
54021	4	335101	7	NULL	NULL	0	NULL	dietary glycine			prevents					hypermetabolic state					NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_299_3_858_s_10	11714869	Importantly, dietary glycine (5%) largely blocked chronic CsA-induced activation of Kupffer cells, blunted production of PGE2, prevented the hypermetabolic state, and minimized tissue hypoxia.	transcription
54022	5	335101	7	NULL	NULL	0	NULL	dietary glycine			minimize					tissue hypoxia					NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_299_3_858_s_10	11714869	Importantly, dietary glycine (5%) largely blocked chronic CsA-induced activation of Kupffer cells, blunted production of PGE2, prevented the hypermetabolic state, and minimized tissue hypoxia.	transcription
54024	1	335102	5	NULL	NULL	0	NULL	disulphide bridge			is formed between					plasminogen			P4 (cysteine);;P 5 (cysteine)		NULL		0	NULL	NULL	NULL	gw60_structure_6_9_1195_s_227	9753698	The following P 3 and P 4 glycine residues of the plasminogen activation loop must fold back to allow disulphide bridge formation between P4 (cysteine) and P 5 (cysteine) of plasminogen (  Figure 4).	transcription
54025	2	335102	5	NULL	NULL	0	NULL	plasminogen 			resides in			P3glycine;;P4 glycine		plasminogen 			activation loop		NULL		0	NULL	NULL	NULL	gw60_structure_6_9_1195_s_227	9753698	The following P 3 and P 4 glycine residues of the plasminogen activation loop must fold back to allow disulphide bridge formation between P4 (cysteine) and P 5 (cysteine) of plasminogen (  Figure 4).	transcription
54026	3	335102	5	NULL	NULL	0	NULL	statement 2		folding back of	allows					statement 1					NULL		0	NULL	NULL	NULL	gw60_structure_6_9_1195_s_227	9753698	The following P 3 and P 4 glycine residues of the plasminogen activation loop must fold back to allow disulphide bridge formation between P4 (cysteine) and P 5 (cysteine) of plasminogen (  Figure 4).	transcription
54023	1	335102	7	NULL	NULL	0	NULL	plasminogen activation loop			allow			P 3 and P 4 glycine residues		plasminogen			disulphide bridge formation between P4 (cysteine) and P 5 (cysteine)		NULL		0	NULL	NULL	NULL	gw60_structure_6_9_1195_s_227	9753698	The following P 3 and P 4 glycine residues of the plasminogen activation loop must fold back to allow disulphide bridge formation between P4 (cysteine) and P 5 (cysteine) of plasminogen (  Figure 4).	transcription
54032	1	335109	7	NULL	NULL	0	NULL	CO-			bind					DNA					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_4_2333_s_78	12433917	For the measurement of DNA binding of CO-, imidazole-and CN -bound deltaP3R4 CooA at pH 9.5, the following assay buffer (high pH anisotropy buffer) was used: 40 mM glycine-NaOH, pH 9.5, 6 mM CaCl2, 50 mM KCl, 5% (v/v) glycerol, and 5 mM dithiothreitol.	transcription
54033	2	335109	7	NULL	NULL	0	NULL	imidazole			bind					deltaP3R4 CooA					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_4_2333_s_78	12433917	For the measurement of DNA binding of CO-, imidazole-and CN -bound deltaP3R4 CooA at pH 9.5, the following assay buffer (high pH anisotropy buffer) was used: 40 mM glycine-NaOH, pH 9.5, 6 mM CaCl2, 50 mM KCl, 5% (v/v) glycerol, and 5 mM dithiothreitol.	transcription
54034	3	335109	7	NULL	NULL	0	NULL	CN			bind					deltaP3R4 CooA					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_4_2333_s_78	12433917	For the measurement of DNA binding of CO-, imidazole-and CN -bound deltaP3R4 CooA at pH 9.5, the following assay buffer (high pH anisotropy buffer) was used: 40 mM glycine-NaOH, pH 9.5, 6 mM CaCl2, 50 mM KCl, 5% (v/v) glycerol, and 5 mM dithiothreitol.	transcription
53576	1	335110	5	NULL	NULL	0	NULL	(2 S,1' S,2' S)-2-(carboxycyclopropyl)-glycine	NULL		is a type of	NULL				group II selective mGluR agonist	NULL				NULL		0	NULL	NULL	NULL	gw70_jneurosci_25_40_9213_s_265	16207881	Application of the group II selective mGluR agonist (2 S,1' S,2' S)-2-(carboxycyclopropyl)-glycine (20 muM) did not depress EPSCs evoked by stimulation at CA1 stratum radiatum (102  plus-or-minus  7% of control;  n = 5 from 5 animals), verifying that the currents were not contaminated by pp inputs.	transcription
53577	2	335110	5	NULL	NULL	0	NULL	EPSCs	NULL		is evoked by	NULL				CA1 stratum radiatum	NULL	stimulation of			NULL		0	NULL	NULL	NULL	gw70_jneurosci_25_40_9213_s_265	16207881	Application of the group II selective mGluR agonist (2 S,1' S,2' S)-2-(carboxycyclopropyl)-glycine (20 muM) did not depress EPSCs evoked by stimulation at CA1 stratum radiatum (102  plus-or-minus  7% of control;  n = 5 from 5 animals), verifying that the currents were not contaminated by pp inputs.	transcription
53578	3	335110	5	NULL	NULL	0	NULL	(2 S,1' S,2' S)-2-(carboxycyclopropyl)-glycine	NULL		does not depress	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_jneurosci_25_40_9213_s_265	16207881	Application of the group II selective mGluR agonist (2 S,1' S,2' S)-2-(carboxycyclopropyl)-glycine (20 muM) did not depress EPSCs evoked by stimulation at CA1 stratum radiatum (102  plus-or-minus  7% of control;  n = 5 from 5 animals), verifying that the currents were not contaminated by pp inputs.	transcription
54035	1	335110	7	NULL	NULL	0	NULL	(2 S,1' S,2' S)-2-(carboxycyclopropyl)-glycine			did not depress					EPSCs					NULL		0	NULL	NULL	NULL	gw70_jneurosci_25_40_9213_s_265	16207881	Application of the group II selective mGluR agonist (2 S,1' S,2' S)-2-(carboxycyclopropyl)-glycine (20 muM) did not depress EPSCs evoked by stimulation at CA1 stratum radiatum (102  plus-or-minus  7% of control;  n = 5 from 5 animals), verifying that the currents were not contaminated by pp inputs.	transcription
54036	2	335110	7	NULL	NULL	0	NULL	statement 1			evoked by					CA1 stratum radiatum		stimulation at			NULL		NULL	NULL	NULL	NULL	gw70_jneurosci_25_40_9213_s_265	16207881	Application of the group II selective mGluR agonist (2 S,1' S,2' S)-2-(carboxycyclopropyl)-glycine (20 muM) did not depress EPSCs evoked by stimulation at CA1 stratum radiatum (102  plus-or-minus  7% of control;  n = 5 from 5 animals), verifying that the currents were not contaminated by pp inputs.	transcription
54037	3	335110	7	NULL	NULL	0	NULL	(2 S,1' S,2' S)-2-(carboxycyclopropyl)-glycine			is a type of					group II selective mGluR agonist					NULL		NULL	NULL	NULL	NULL	gw70_jneurosci_25_40_9213_s_265	16207881	Application of the group II selective mGluR agonist (2 S,1' S,2' S)-2-(carboxycyclopropyl)-glycine (20 muM) did not depress EPSCs evoked by stimulation at CA1 stratum radiatum (102  plus-or-minus  7% of control;  n = 5 from 5 animals), verifying that the currents were not contaminated by pp inputs.	transcription
53579	1	335113	5	NULL	NULL	0	NULL	IGF-1R-LexA construct	NULL		is expressed with	NULL				proline-glycine spacer	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_36_33419_s_35	11445579	Expression of the IGF-1R-LexA construct with a proline-glycine spacer resulted in the highest autokinase activity and the strongest interaction with p85alpha (PCR was performed with the following oligonucleotides: sense primer with an  EcoRI/ SmaI adaptor: 5''-TCCGGAATTCCCGGGGAGAAAGAGAAATAACAGCAGGCTGG3-'', reverse primer with an  SalI/ BamHI adaptor: 5''-TCCGGTCGACGGATCCAAGGATCAGCAGGTCGAA-3'').	transcription
53580	2	335113	5	NULL	NULL	0	NULL	statement 1	NULL		results in	NULL				autokinase activity	NULL	highest			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_36_33419_s_35	11445579	Expression of the IGF-1R-LexA construct with a proline-glycine spacer resulted in the highest autokinase activity and the strongest interaction with p85alpha (PCR was performed with the following oligonucleotides: sense primer with an  EcoRI/ SmaI adaptor: 5''-TCCGGAATTCCCGGGGAGAAAGAGAAATAACAGCAGGCTGG3-'', reverse primer with an  SalI/ BamHI adaptor: 5''-TCCGGTCGACGGATCCAAGGATCAGCAGGTCGAA-3'').	transcription
53581	3	335113	5	NULL	NULL	0	NULL	statement 1	NULL		results in	NULL				p85alpha	NULL	strongest interaction with			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_36_33419_s_35	11445579	Expression of the IGF-1R-LexA construct with a proline-glycine spacer resulted in the highest autokinase activity and the strongest interaction with p85alpha (PCR was performed with the following oligonucleotides: sense primer with an  EcoRI/ SmaI adaptor: 5''-TCCGGAATTCCCGGGGAGAAAGAGAAATAACAGCAGGCTGG3-'', reverse primer with an  SalI/ BamHI adaptor: 5''-TCCGGTCGACGGATCCAAGGATCAGCAGGTCGAA-3'').	transcription
54038	1	335113	7	NULL	NULL	0	NULL	IGF-1R-LexA construct			is expressed with					proline-glycine spacer					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_36_33419_s_35	11445579	Expression of the IGF-1R-LexA construct with a proline-glycine spacer resulted in the highest autokinase activity and the strongest interaction with p85alpha (PCR was performed with the following oligonucleotides: sense primer with an  EcoRI/ SmaI adaptor: 5''-TCCGGAATTCCCGGGGAGAAAGAGAAATAACAGCAGGCTGG3-'', reverse primer with an  SalI/ BamHI adaptor: 5''-TCCGGTCGACGGATCCAAGGATCAGCAGGTCGAA-3'').	transcription
54039	2	335113	7	NULL	NULL	0	NULL	statement 1			results in					 autokinase 		highest activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_36_33419_s_35	11445579	Expression of the IGF-1R-LexA construct with a proline-glycine spacer resulted in the highest autokinase activity and the strongest interaction with p85alpha (PCR was performed with the following oligonucleotides: sense primer with an  EcoRI/ SmaI adaptor: 5''-TCCGGAATTCCCGGGGAGAAAGAGAAATAACAGCAGGCTGG3-'', reverse primer with an  SalI/ BamHI adaptor: 5''-TCCGGTCGACGGATCCAAGGATCAGCAGGTCGAA-3'').	transcription
54040	3	335113	7	NULL	NULL	0	NULL	statement 1			interacts with		strongly			 p85alpha					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_36_33419_s_35	11445579	Expression of the IGF-1R-LexA construct with a proline-glycine spacer resulted in the highest autokinase activity and the strongest interaction with p85alpha (PCR was performed with the following oligonucleotides: sense primer with an  EcoRI/ SmaI adaptor: 5''-TCCGGAATTCCCGGGGAGAAAGAGAAATAACAGCAGGCTGG3-'', reverse primer with an  SalI/ BamHI adaptor: 5''-TCCGGTCGACGGATCCAAGGATCAGCAGGTCGAA-3'').	transcription
53582	1	335114	5	NULL	NULL	0	NULL	NMDA receptor	NULL	activation of	is dependent on	NULL				glycine	NULL				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_302_1_163_s_184	12065713	As depicted in Fig.  5A, the glycine-dependent activation of the NMDA receptor exhibited an EC50 of 0.8  plus-or-minus  0.1 muM ( n = 5) that was not significantly changed by the presence of 20 muM N20C in the medium (EC50 = 1.1  plus-or-minus  0.3 muM,  n = 5).	transcription
54041	1	335114	7	NULL	NULL	0	NULL	NMDA receptor		activation of	depends on					glycine					NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_302_1_163_s_184	12065713	As depicted in Fig.  5A, the glycine-dependent activation of the NMDA receptor exhibited an EC50 of 0.8  plus-or-minus  0.1 muM ( n = 5) that was not significantly changed by the presence of 20 muM N20C in the medium (EC50 = 1.1  plus-or-minus  0.3 muM,  n = 5).	transcription
53583	1	335116	5	NULL	NULL	0	NULL	glycine	NULL		activates	NULL				NMDA receptor	NULL		glycine-binding site		NULL		0	NULL	NULL	NULL	gw70_nature_438_7071_1162_s_127	16372011	Slices were superfused at  33   1  degrees C with bicarbonate-buffered solution (for ischaemia experiments) containing  126 mM NaCl, 24 mM NaHCO3, 1 mM NaH2PO4, 2.5 mM KCl, 2 mM MgCl2, 2.5 mM CaCl2, 10 mM glucose, 0.1 mM glycine (which activates the NMDA receptor glycine-binding  site) and 0.005 mM strychnine (which blocks glycine receptors), bubbled with 95%  O2, 5% CO2 (pH 7.4); or at 24   1  degrees C with HEPES-buffered solution (for non-ischaemia experiments) containing  144 mM NaCl, 2.5 mM KCl, 2 mM MgCl2, 10 mM HEPES, 1 mM NaH2PO4, 2.5 mM CaCl2, 10 mM glucose, 0.1 mM glycine and 0.005 mM strychnine, with the pH set to 7.4 using  NaOH.	transcription
53584	2	335116	5	NULL	NULL	0	NULL	strychnine	NULL		blocks	NULL				glycine receptors	NULL				NULL		0	NULL	NULL	NULL	gw70_nature_438_7071_1162_s_127	16372011	Slices were superfused at  33   1  degrees C with bicarbonate-buffered solution (for ischaemia experiments) containing  126 mM NaCl, 24 mM NaHCO3, 1 mM NaH2PO4, 2.5 mM KCl, 2 mM MgCl2, 2.5 mM CaCl2, 10 mM glucose, 0.1 mM glycine (which activates the NMDA receptor glycine-binding  site) and 0.005 mM strychnine (which blocks glycine receptors), bubbled with 95%  O2, 5% CO2 (pH 7.4); or at 24   1  degrees C with HEPES-buffered solution (for non-ischaemia experiments) containing  144 mM NaCl, 2.5 mM KCl, 2 mM MgCl2, 10 mM HEPES, 1 mM NaH2PO4, 2.5 mM CaCl2, 10 mM glucose, 0.1 mM glycine and 0.005 mM strychnine, with the pH set to 7.4 using  NaOH.	transcription
54042	1	335116	7	NULL	NULL	0	NULL	bicarbonate-buffered solution			activates					NMDA receptor			glycine-binding site		NULL		0	NULL	NULL	NULL	gw70_nature_438_7071_1162_s_127	16372011	Slices were superfused at  33   1  degrees C with bicarbonate-buffered solution (for ischaemia experiments) containing  126 mM NaCl, 24 mM NaHCO3, 1 mM NaH2PO4, 2.5 mM KCl, 2 mM MgCl2, 2.5 mM CaCl2, 10 mM glucose, 0.1 mM glycine (which activates the NMDA receptor glycine-binding  site) and 0.005 mM strychnine (which blocks glycine receptors), bubbled with 95%  O2, 5% CO2 (pH 7.4); or at 24   1  degrees C with HEPES-buffered solution (for non-ischaemia experiments) containing  144 mM NaCl, 2.5 mM KCl, 2 mM MgCl2, 10 mM HEPES, 1 mM NaH2PO4, 2.5 mM CaCl2, 10 mM glucose, 0.1 mM glycine and 0.005 mM strychnine, with the pH set to 7.4 using  NaOH.	transcription
54043	2	335116	7	NULL	NULL	0	NULL	strychnine			block					glycine receptors					NULL		0	NULL	NULL	NULL	gw70_nature_438_7071_1162_s_127	16372011	Slices were superfused at  33   1  degrees C with bicarbonate-buffered solution (for ischaemia experiments) containing  126 mM NaCl, 24 mM NaHCO3, 1 mM NaH2PO4, 2.5 mM KCl, 2 mM MgCl2, 2.5 mM CaCl2, 10 mM glucose, 0.1 mM glycine (which activates the NMDA receptor glycine-binding  site) and 0.005 mM strychnine (which blocks glycine receptors), bubbled with 95%  O2, 5% CO2 (pH 7.4); or at 24   1  degrees C with HEPES-buffered solution (for non-ischaemia experiments) containing  144 mM NaCl, 2.5 mM KCl, 2 mM MgCl2, 10 mM HEPES, 1 mM NaH2PO4, 2.5 mM CaCl2, 10 mM glucose, 0.1 mM glycine and 0.005 mM strychnine, with the pH set to 7.4 using  NaOH.	transcription
53585	1	335117	5	NULL	NULL	0	NULL	glycine	NULL		reduces	NULL				NFPS	NULL	binding of			NULL		0	NULL	NULL	NULL	gw70_neuropharmacology_45_5_585_s_135	12941372	As illustrated in  Fig. 4A by saturation plot and Scatchard transformation, glycine reduced maximal [3]NFPS binding (58 plus-or-minus 5% at 1 mM glycine;  P<0.05;  t-test paired, two-tailed) without significantly changing the affinity of [3]NFPS for its binding site ( Kd=4.2 plus-or-minus 0.4 nM, compared to 6.2 plus-or-minus 2.3 nM for control).	transcription
53586	2	335117	5	NULL	NULL	0	NULL	statement 1	NULL		without changing	NULL	significantly			NFPS	NULL	affinity of			NULL		0	NULL	NULL	NULL	gw70_neuropharmacology_45_5_585_s_135	12941372	As illustrated in  Fig. 4A by saturation plot and Scatchard transformation, glycine reduced maximal [3]NFPS binding (58 plus-or-minus 5% at 1 mM glycine;  P<0.05;  t-test paired, two-tailed) without significantly changing the affinity of [3]NFPS for its binding site ( Kd=4.2 plus-or-minus 0.4 nM, compared to 6.2 plus-or-minus 2.3 nM for control).	transcription
54044	1	335117	7	NULL	NULL	0	NULL	glycine			reduce					NFPS		binding of			NULL		0	NULL	NULL	NULL	gw70_neuropharmacology_45_5_585_s_135	12941372	As illustrated in  Fig. 4A by saturation plot and Scatchard transformation, glycine reduced maximal [3]NFPS binding (58 plus-or-minus 5% at 1 mM glycine;  P<0.05;  t-test paired, two-tailed) without significantly changing the affinity of [3]NFPS for its binding site ( Kd=4.2 plus-or-minus 0.4 nM, compared to 6.2 plus-or-minus 2.3 nM for control).	transcription
53587	1	335118	5	NULL	NULL	0	NULL	deoxyhemoglobin	NULL		bind	NULL	avidly			CO	NULL				NULL		0	NULL	NULL	NULL	gw60_circulationres_83_5_568_s_93	9734480	The lower chamber contained 5 muCi of [2-14C]L-glycine, a heme precursor, and the upper chamber contained a solution of deoxyhemoglobin (15 mumol/L), which is known to avidly bind CO. Aortas were removed from rats at various times after surgery, trimmed of adventitial tissue, and transferred into the lower chamber containing [2-14C]L-glycine in oxygenated Krebs-Henseleit buffer (1:20 [vol/vol]) containing (mmol/L) NaCl 118, KCl 4.7, KH2PO4 1.2, MgSO4 .	transcription
54045	1	335118	7	NULL	NULL	0	NULL	deoxyhemoglobin			bind		avidly			CO					NULL		0	NULL	NULL	NULL	gw60_circulationres_83_5_568_s_93	9734480	The lower chamber contained 5 muCi of [2-14C]L-glycine, a heme precursor, and the upper chamber contained a solution of deoxyhemoglobin (15 mumol/L), which is known to avidly bind CO. Aortas were removed from rats at various times after surgery, trimmed of adventitial tissue, and transferred into the lower chamber containing [2-14C]L-glycine in oxygenated Krebs-Henseleit buffer (1:20 [vol/vol]) containing (mmol/L) NaCl 118, KCl 4.7, KH2PO4 1.2, MgSO4 .	transcription
53588	1	335119	5	NULL	NULL	0	NULL	glycine	NULL		is mutated to	NULL		position 269		cysteine	NULL		position 269		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_37_21659_s_138	7665581	Mutation of the glycine residues at positions  269 and 271 to cysteine and arginine respectively, had no effect on ATP  binding, although both of these mutations resulted in decreased  selenium labeling of 5``-deiodinase ( Fig. 4 b  and data  not shown), suggesting that the glycine residues at these positions  have roles in normal selenophosphate synthetase activity other than ATP  binding.	transcription
53589	2	335119	5	NULL	NULL	0	NULL	glycine	NULL		is mutated to	NULL		position 271		arginine	NULL		position 271		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_37_21659_s_138	7665581	Mutation of the glycine residues at positions  269 and 271 to cysteine and arginine respectively, had no effect on ATP  binding, although both of these mutations resulted in decreased  selenium labeling of 5``-deiodinase ( Fig. 4 b  and data  not shown), suggesting that the glycine residues at these positions  have roles in normal selenophosphate synthetase activity other than ATP  binding.	transcription
53590	3	335119	5	NULL	NULL	0	NULL	statement 1	NULL		does not effect	NULL				ATP	NULL	binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_37_21659_s_138	7665581	Mutation of the glycine residues at positions  269 and 271 to cysteine and arginine respectively, had no effect on ATP  binding, although both of these mutations resulted in decreased  selenium labeling of 5``-deiodinase ( Fig. 4 b  and data  not shown), suggesting that the glycine residues at these positions  have roles in normal selenophosphate synthetase activity other than ATP  binding.	transcription
53591	4	335119	5	NULL	NULL	0	NULL	statement 2	NULL		does not effect	NULL				ATP	NULL	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_37_21659_s_138	7665581	Mutation of the glycine residues at positions  269 and 271 to cysteine and arginine respectively, had no effect on ATP  binding, although both of these mutations resulted in decreased  selenium labeling of 5``-deiodinase ( Fig. 4 b  and data  not shown), suggesting that the glycine residues at these positions  have roles in normal selenophosphate synthetase activity other than ATP  binding.	transcription
53592	5	335119	5	NULL	NULL	0	NULL	glycine	NULL		plays a role in	NULL		position 269		selenophosphate synthetase activity	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_37_21659_s_138	7665581	Mutation of the glycine residues at positions  269 and 271 to cysteine and arginine respectively, had no effect on ATP  binding, although both of these mutations resulted in decreased  selenium labeling of 5``-deiodinase ( Fig. 4 b  and data  not shown), suggesting that the glycine residues at these positions  have roles in normal selenophosphate synthetase activity other than ATP  binding.	transcription
53593	6	335119	5	NULL	NULL	0	NULL	glycine	NULL		plays a role in	NULL		position 271		selenophosphate synthetase activity	NULL				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_37_21659_s_138	7665581	Mutation of the glycine residues at positions  269 and 271 to cysteine and arginine respectively, had no effect on ATP  binding, although both of these mutations resulted in decreased  selenium labeling of 5``-deiodinase ( Fig. 4 b  and data  not shown), suggesting that the glycine residues at these positions  have roles in normal selenophosphate synthetase activity other than ATP  binding.	transcription
54046	1	335119	7	NULL	NULL	0	NULL				mutated to			glycine residue at position 269					cysteine at position 269		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_37_21659_s_138	7665581	Mutation of the glycine residues at positions  269 and 271 to cysteine and arginine respectively, had no effect on ATP  binding, although both of these mutations resulted in decreased  selenium labeling of 5``-deiodinase ( Fig. 4 b  and data  not shown), suggesting that the glycine residues at these positions  have roles in normal selenophosphate synthetase activity other than ATP  binding.	transcription
54047	2	335119	7	NULL	NULL	0	NULL	statement 1			does not effect					ATP		binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_37_21659_s_138	7665581	Mutation of the glycine residues at positions  269 and 271 to cysteine and arginine respectively, had no effect on ATP  binding, although both of these mutations resulted in decreased  selenium labeling of 5``-deiodinase ( Fig. 4 b  and data  not shown), suggesting that the glycine residues at these positions  have roles in normal selenophosphate synthetase activity other than ATP  binding.	transcription
54048	3	335119	7	NULL	NULL	0	NULL				mutated to			glycine residue at position 271					arginine at position 271		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_37_21659_s_138	7665581	Mutation of the glycine residues at positions  269 and 271 to cysteine and arginine respectively, had no effect on ATP  binding, although both of these mutations resulted in decreased  selenium labeling of 5``-deiodinase ( Fig. 4 b  and data  not shown), suggesting that the glycine residues at these positions  have roles in normal selenophosphate synthetase activity other than ATP  binding.	transcription
54049	4	335119	7	NULL	NULL	0	NULL	statement 3			does not effect					ATP		binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_37_21659_s_138	7665581	Mutation of the glycine residues at positions  269 and 271 to cysteine and arginine respectively, had no effect on ATP  binding, although both of these mutations resulted in decreased  selenium labeling of 5``-deiodinase ( Fig. 4 b  and data  not shown), suggesting that the glycine residues at these positions  have roles in normal selenophosphate synthetase activity other than ATP  binding.	transcription
54050	5	335119	7	NULL	NULL	0	NULL	statement 1			decrease					5``-deiodinase		selenium labeling of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_37_21659_s_138	7665581	Mutation of the glycine residues at positions  269 and 271 to cysteine and arginine respectively, had no effect on ATP  binding, although both of these mutations resulted in decreased  selenium labeling of 5``-deiodinase ( Fig. 4 b  and data  not shown), suggesting that the glycine residues at these positions  have roles in normal selenophosphate synthetase activity other than ATP  binding.	transcription
54051	6	335119	7	NULL	NULL	0	NULL	statement 3			decrease					5``-deiodinase		selenium labeling of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_37_21659_s_138	7665581	Mutation of the glycine residues at positions  269 and 271 to cysteine and arginine respectively, had no effect on ATP  binding, although both of these mutations resulted in decreased  selenium labeling of 5``-deiodinase ( Fig. 4 b  and data  not shown), suggesting that the glycine residues at these positions  have roles in normal selenophosphate synthetase activity other than ATP  binding.	transcription
54052	7	335119	7	NULL	NULL	0	NULL				play a role in			glycine residue at position 269 		selenophosphate synthetase 		normal;;activity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_37_21659_s_138	7665581	Mutation of the glycine residues at positions  269 and 271 to cysteine and arginine respectively, had no effect on ATP  binding, although both of these mutations resulted in decreased  selenium labeling of 5``-deiodinase ( Fig. 4 b  and data  not shown), suggesting that the glycine residues at these positions  have roles in normal selenophosphate synthetase activity other than ATP  binding.	transcription
54053	8	335119	7	NULL	NULL	0	NULL				play a role in			glycine residue at position 271		selenophosphate synthetase 		normal;;activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_37_21659_s_138	7665581	Mutation of the glycine residues at positions  269 and 271 to cysteine and arginine respectively, had no effect on ATP  binding, although both of these mutations resulted in decreased  selenium labeling of 5``-deiodinase ( Fig. 4 b  and data  not shown), suggesting that the glycine residues at these positions  have roles in normal selenophosphate synthetase activity other than ATP  binding.	transcription
54054	9	335119	7	NULL	NULL	0	NULL	statement 2			suggest					statement 7					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_37_21659_s_138	7665581	Mutation of the glycine residues at positions  269 and 271 to cysteine and arginine respectively, had no effect on ATP  binding, although both of these mutations resulted in decreased  selenium labeling of 5``-deiodinase ( Fig. 4 b  and data  not shown), suggesting that the glycine residues at these positions  have roles in normal selenophosphate synthetase activity other than ATP  binding.	transcription
54055	10	335119	7	NULL	NULL	0	NULL	statement 4			suggests					statement 8					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_37_21659_s_138	7665581	Mutation of the glycine residues at positions  269 and 271 to cysteine and arginine respectively, had no effect on ATP  binding, although both of these mutations resulted in decreased  selenium labeling of 5``-deiodinase ( Fig. 4 b  and data  not shown), suggesting that the glycine residues at these positions  have roles in normal selenophosphate synthetase activity other than ATP  binding.	transcription
53594	1	335120	5	NULL	NULL	0	NULL	GlyRs	NULL		decreases	NULL		D148E		strychnine	NULL	affinity of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_mol-pharmacol_44_1_8393521_s_14	8393521	The D148E GlyRs showed a 1 order of magnitude decrease in strychnine affinity  (Kd, 8.1 +/- 1.4 nM versus 82 +/- 21 nM), without any change in the glycine  displacement of strychnine binding (Ki, 25 +/- 5 microM versus 29 +/-  8 microM) or glycine activation of chloride currents (EC50, 27 +/- 6 microM  versus 20 +/- 1 microM).	transcription
53595	2	335120	5	NULL	NULL	0	NULL	glycine	NULL		activates	NULL				chloride currents	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_mol-pharmacol_44_1_8393521_s_14	8393521	The D148E GlyRs showed a 1 order of magnitude decrease in strychnine affinity  (Kd, 8.1 +/- 1.4 nM versus 82 +/- 21 nM), without any change in the glycine  displacement of strychnine binding (Ki, 25 +/- 5 microM versus 29 +/-  8 microM) or glycine activation of chloride currents (EC50, 27 +/- 6 microM  versus 20 +/- 1 microM).	transcription
53596	3	335120	5	NULL	NULL	0	NULL	statement 1	NULL		does not change	NULL				statement 2	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_mol-pharmacol_44_1_8393521_s_14	8393521	The D148E GlyRs showed a 1 order of magnitude decrease in strychnine affinity  (Kd, 8.1 +/- 1.4 nM versus 82 +/- 21 nM), without any change in the glycine  displacement of strychnine binding (Ki, 25 +/- 5 microM versus 29 +/-  8 microM) or glycine activation of chloride currents (EC50, 27 +/- 6 microM  versus 20 +/- 1 microM).	transcription
53597	4	335120	5	NULL	NULL	0	NULL	glycine	NULL		displaced in	NULL				strychnine	NULL	binding of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_mol-pharmacol_44_1_8393521_s_14	8393521	The D148E GlyRs showed a 1 order of magnitude decrease in strychnine affinity  (Kd, 8.1 +/- 1.4 nM versus 82 +/- 21 nM), without any change in the glycine  displacement of strychnine binding (Ki, 25 +/- 5 microM versus 29 +/-  8 microM) or glycine activation of chloride currents (EC50, 27 +/- 6 microM  versus 20 +/- 1 microM).	transcription
53598	5	335120	5	NULL	NULL	0	NULL	statement 1	NULL		does not change	NULL				statement 4	NULL				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_mol-pharmacol_44_1_8393521_s_14	8393521	The D148E GlyRs showed a 1 order of magnitude decrease in strychnine affinity  (Kd, 8.1 +/- 1.4 nM versus 82 +/- 21 nM), without any change in the glycine  displacement of strychnine binding (Ki, 25 +/- 5 microM versus 29 +/-  8 microM) or glycine activation of chloride currents (EC50, 27 +/- 6 microM  versus 20 +/- 1 microM).	transcription
54056	1	335120	7	NULL	NULL	0	NULL	GlyRs			decrease			D148E		strychnine		affinity of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_mol-pharmacol_44_1_8393521_s_14	8393521	The D148E GlyRs showed a 1 order of magnitude decrease in strychnine affinity  (Kd, 8.1 +/- 1.4 nM versus 82 +/- 21 nM), without any change in the glycine  displacement of strychnine binding (Ki, 25 +/- 5 microM versus 29 +/-  8 microM) or glycine activation of chloride currents (EC50, 27 +/- 6 microM  versus 20 +/- 1 microM).	transcription
54057	2	335120	7	NULL	NULL	0	NULL	glycine			activate					chloride currents					NULL		0	NULL	NULL	NULL	abs-batch0650-0679_mol-pharmacol_44_1_8393521_s_14	8393521	The D148E GlyRs showed a 1 order of magnitude decrease in strychnine affinity  (Kd, 8.1 +/- 1.4 nM versus 82 +/- 21 nM), without any change in the glycine  displacement of strychnine binding (Ki, 25 +/- 5 microM versus 29 +/-  8 microM) or glycine activation of chloride currents (EC50, 27 +/- 6 microM  versus 20 +/- 1 microM).	transcription
54058	3	335120	7	NULL	NULL	0	NULL	GlyRs			does not change			D148E		statement 2					NULL		0	NULL	NULL	NULL	abs-batch0650-0679_mol-pharmacol_44_1_8393521_s_14	8393521	The D148E GlyRs showed a 1 order of magnitude decrease in strychnine affinity  (Kd, 8.1 +/- 1.4 nM versus 82 +/- 21 nM), without any change in the glycine  displacement of strychnine binding (Ki, 25 +/- 5 microM versus 29 +/-  8 microM) or glycine activation of chloride currents (EC50, 27 +/- 6 microM  versus 20 +/- 1 microM).	transcription
53599	1	335122	5	NULL	NULL	0	NULL	CCBD	NULL		is	NULL				central cell-binding domain	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_260_2_449_s_23	12921745	The central cell-binding domain (CCBD) of fibronectin contains the RGD (Arginine-Glycine-Aspartic  acid) sequence and an adjacent site that acts in synergy with RGD to allow  5 1-dependent  cell spreading and cell migration [  Mould et al 1997 and   Obara and Yoshizato 1995].	transcription
53600	2	335122	5	NULL	NULL	0	NULL	RGD	NULL		is	NULL				Arginine-Glycine-Aspartic acid	NULL				NULL		0	NULL	NULL	NULL	gw70_devbiol_260_2_449_s_23	12921745	The central cell-binding domain (CCBD) of fibronectin contains the RGD (Arginine-Glycine-Aspartic  acid) sequence and an adjacent site that acts in synergy with RGD to allow  5 1-dependent  cell spreading and cell migration [  Mould et al 1997 and   Obara and Yoshizato 1995].	transcription
53601	3	335122	5	NULL	NULL	0	NULL	fibronectin	NULL		contains	NULL		CCBD		fibronectin \t	NULL		RGD		NULL		NULL	NULL	NULL	NULL	gw70_devbiol_260_2_449_s_23	12921745	The central cell-binding domain (CCBD) of fibronectin contains the RGD (Arginine-Glycine-Aspartic  acid) sequence and an adjacent site that acts in synergy with RGD to allow  5 1-dependent  cell spreading and cell migration [  Mould et al 1997 and   Obara and Yoshizato 1995].	transcription
53602	4	335122	5	NULL	NULL	0	NULL	fibronectin \t	NULL	adjacent site of	acts in synergy with	NULL		RGD		fibronectin \t	NULL		RGD		NULL		NULL	NULL	NULL	NULL	gw70_devbiol_260_2_449_s_23	12921745	The central cell-binding domain (CCBD) of fibronectin contains the RGD (Arginine-Glycine-Aspartic  acid) sequence and an adjacent site that acts in synergy with RGD to allow  5 1-dependent  cell spreading and cell migration [  Mould et al 1997 and   Obara and Yoshizato 1995].	transcription
53603	5	335122	5	NULL	NULL	0	NULL	statement 4	NULL		allows	NULL				cell	NULL	spreading of			NULL		0	NULL	NULL	NULL	gw70_devbiol_260_2_449_s_23	12921745	The central cell-binding domain (CCBD) of fibronectin contains the RGD (Arginine-Glycine-Aspartic  acid) sequence and an adjacent site that acts in synergy with RGD to allow  5 1-dependent  cell spreading and cell migration [  Mould et al 1997 and   Obara and Yoshizato 1995].	transcription
53604	6	335122	5	NULL	NULL	0	NULL	statement 4	NULL		allows	NULL				cell	NULL	migration of			NULL		0	NULL	NULL	NULL	gw70_devbiol_260_2_449_s_23	12921745	The central cell-binding domain (CCBD) of fibronectin contains the RGD (Arginine-Glycine-Aspartic  acid) sequence and an adjacent site that acts in synergy with RGD to allow  5 1-dependent  cell spreading and cell migration [  Mould et al 1997 and   Obara and Yoshizato 1995].	transcription
54059	1	335122	7	NULL	NULL	0	NULL	fibronectin			contains			CCBD					RGD sequence 		NULL		0	NULL	NULL	NULL	gw70_devbiol_260_2_449_s_23	12921745	The central cell-binding domain (CCBD) of fibronectin contains the RGD (Arginine-Glycine-Aspartic  acid) sequence and an adjacent site that acts in synergy with RGD to allow  5 1-dependent  cell spreading and cell migration [  Mould et al 1997 and   Obara and Yoshizato 1995].	transcription
54060	2	335122	7	NULL	NULL	0	NULL	statement 1			allow					cell spreading					NULL		0	NULL	NULL	NULL	gw70_devbiol_260_2_449_s_23	12921745	The central cell-binding domain (CCBD) of fibronectin contains the RGD (Arginine-Glycine-Aspartic  acid) sequence and an adjacent site that acts in synergy with RGD to allow  5 1-dependent  cell spreading and cell migration [  Mould et al 1997 and   Obara and Yoshizato 1995].	transcription
54061	3	335122	7	NULL	NULL	0	NULL	statement 1			allow					cell migration					NULL		0	NULL	NULL	NULL	gw70_devbiol_260_2_449_s_23	12921745	The central cell-binding domain (CCBD) of fibronectin contains the RGD (Arginine-Glycine-Aspartic  acid) sequence and an adjacent site that acts in synergy with RGD to allow  5 1-dependent  cell spreading and cell migration [  Mould et al 1997 and   Obara and Yoshizato 1995].	transcription
54062	4	335122	7	NULL	NULL	0	NULL	CCBD			is					central cell-binding domain					NULL		0	NULL	NULL	NULL	gw70_devbiol_260_2_449_s_23	12921745	The central cell-binding domain (CCBD) of fibronectin contains the RGD (Arginine-Glycine-Aspartic  acid) sequence and an adjacent site that acts in synergy with RGD to allow  5 1-dependent  cell spreading and cell migration [  Mould et al 1997 and   Obara and Yoshizato 1995].	transcription
54063	5	335122	7	NULL	NULL	0	NULL	RGD			is					Arginine-Glycine-Aspartic acid					NULL		0	NULL	NULL	NULL	gw70_devbiol_260_2_449_s_23	12921745	The central cell-binding domain (CCBD) of fibronectin contains the RGD (Arginine-Glycine-Aspartic  acid) sequence and an adjacent site that acts in synergy with RGD to allow  5 1-dependent  cell spreading and cell migration [  Mould et al 1997 and   Obara and Yoshizato 1995].	transcription
53605	1	335123	5	NULL	NULL	0	NULL	HAT	NULL	enzymatic activity of	plays a role in	NULL	critical			X chromosome	NULL	increased transcription of;;male			NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_70_0_81_s_141	11395403	Indeed, mutation of the single underlined glycine (Gly) to  glutamic acid in motif A (Arg/ln-X-X- Gly-X-Glyla; see  Figure 5 D) led to the original discovery of MOF, supporting a critical role for HAT enzymatic  activity in the twofold increased transcription of the male X chromosome (reviewed  in  47,  92).	transcription
54064	1	335123	7	NULL	NULL	0	NULL	HAT		enzymatic activity of	play a critical role in					male X chromosome		increased transcription of			NULL		NULL	NULL	NULL	NULL	gw70_annurevbiochem_70_0_81_s_141	11395403	Indeed, mutation of the single underlined glycine (Gly) to  glutamic acid in motif A (Arg/ln-X-X- Gly-X-Glyla; see  Figure 5 D) led to the original discovery of MOF, supporting a critical role for HAT enzymatic  activity in the twofold increased transcription of the male X chromosome (reviewed  in  47,  92).	transcription
54065	2	335123	7	NULL	NULL	0	NULL				mutated to			Gly in motif A					glutamic acid in motif A		NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_70_0_81_s_141	11395403	Indeed, mutation of the single underlined glycine (Gly) to  glutamic acid in motif A (Arg/ln-X-X- Gly-X-Glyla; see  Figure 5 D) led to the original discovery of MOF, supporting a critical role for HAT enzymatic  activity in the twofold increased transcription of the male X chromosome (reviewed  in  47,  92).	transcription
54066	3	335123	7	NULL	NULL	0	NULL	statement 2			support					statement 1					NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_70_0_81_s_141	11395403	Indeed, mutation of the single underlined glycine (Gly) to  glutamic acid in motif A (Arg/ln-X-X- Gly-X-Glyla; see  Figure 5 D) led to the original discovery of MOF, supporting a critical role for HAT enzymatic  activity in the twofold increased transcription of the male X chromosome (reviewed  in  47,  92).	transcription
54067	4	335123	7	NULL	NULL	0	NULL	Gly			is					glycine					NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_70_0_81_s_141	11395403	Indeed, mutation of the single underlined glycine (Gly) to  glutamic acid in motif A (Arg/ln-X-X- Gly-X-Glyla; see  Figure 5 D) led to the original discovery of MOF, supporting a critical role for HAT enzymatic  activity in the twofold increased transcription of the male X chromosome (reviewed  in  47,  92).	transcription
53606	1	335124	5	NULL	NULL	0	NULL	NMDARs	NULL	internalization of	occurs after	NULL				glycine	NULL	priming of			NULL		0	NULL	NULL	NULL	gw70_nature_422_6929_302_s_138	12646920	To determine whether the internalization of NMDARs after glycine priming was mediated  through clathrin-dependent endocytosis, we made use of a dynamin inhibitory peptide,  QVPSRPNRAP, which competitively binds with the amphiphysin SH3 domain 15 and prevents endocytosis when administered intracellularly 5,  10.	transcription
53607	2	335124	5	NULL	NULL	0	NULL	endocytosis	NULL		is dependent on	NULL				clathrin	NULL				NULL		0	NULL	NULL	NULL	gw70_nature_422_6929_302_s_138	12646920	To determine whether the internalization of NMDARs after glycine priming was mediated  through clathrin-dependent endocytosis, we made use of a dynamin inhibitory peptide,  QVPSRPNRAP, which competitively binds with the amphiphysin SH3 domain 15 and prevents endocytosis when administered intracellularly 5,  10.	transcription
53608	3	335124	5	NULL	NULL	0	NULL	statement 1	NULL		is mediated through	NULL	possibly			statement 2	NULL				NULL		0	NULL	NULL	NULL	gw70_nature_422_6929_302_s_138	12646920	To determine whether the internalization of NMDARs after glycine priming was mediated  through clathrin-dependent endocytosis, we made use of a dynamin inhibitory peptide,  QVPSRPNRAP, which competitively binds with the amphiphysin SH3 domain 15 and prevents endocytosis when administered intracellularly 5,  10.	transcription
53609	4	335124	5	NULL	NULL	0	NULL	QVPSRPNRAP	NULL		is an inhibitory peptide of	NULL				dynamin	NULL				NULL		0	NULL	NULL	NULL	gw70_nature_422_6929_302_s_138	12646920	To determine whether the internalization of NMDARs after glycine priming was mediated  through clathrin-dependent endocytosis, we made use of a dynamin inhibitory peptide,  QVPSRPNRAP, which competitively binds with the amphiphysin SH3 domain 15 and prevents endocytosis when administered intracellularly 5,  10.	transcription
53610	5	335124	5	NULL	NULL	0	NULL		NULL		bind	NULL	competitively	QVPSRPNRAP		amphiphysin	NULL		SH3 domain		NULL		0	NULL	NULL	NULL	gw70_nature_422_6929_302_s_138	12646920	To determine whether the internalization of NMDARs after glycine priming was mediated  through clathrin-dependent endocytosis, we made use of a dynamin inhibitory peptide,  QVPSRPNRAP, which competitively binds with the amphiphysin SH3 domain 15 and prevents endocytosis when administered intracellularly 5,  10.	transcription
53611	6	335124	5	NULL	NULL	0	NULL	statement 5	NULL		prevents	NULL				endocytosis	NULL				NULL		NULL	NULL	NULL	NULL	gw70_nature_422_6929_302_s_138	12646920	To determine whether the internalization of NMDARs after glycine priming was mediated  through clathrin-dependent endocytosis, we made use of a dynamin inhibitory peptide,  QVPSRPNRAP, which competitively binds with the amphiphysin SH3 domain 15 and prevents endocytosis when administered intracellularly 5,  10.	transcription
54068	1	335124	7	NULL	NULL	0	NULL	dynamin inhibitory peptide			bind		competitively			amphiphysin			SH3 domain		NULL		0	NULL	NULL	NULL	gw70_nature_422_6929_302_s_138	12646920	To determine whether the internalization of NMDARs after glycine priming was mediated  through clathrin-dependent endocytosis, we made use of a dynamin inhibitory peptide,  QVPSRPNRAP, which competitively binds with the amphiphysin SH3 domain 15 and prevents endocytosis when administered intracellularly 5,  10.	transcription
54069	2	335124	7	NULL	NULL	0	NULL	statement 1			prevents					endocytosis 					NULL	intracellularly	NULL	NULL	NULL	NULL	gw70_nature_422_6929_302_s_138	12646920	To determine whether the internalization of NMDARs after glycine priming was mediated  through clathrin-dependent endocytosis, we made use of a dynamin inhibitory peptide,  QVPSRPNRAP, which competitively binds with the amphiphysin SH3 domain 15 and prevents endocytosis when administered intracellularly 5,  10.	transcription
54070	3	335124	7	NULL	NULL	0	NULL	 NMDARs		internalization of	occurs after					 glycine		priming of			NULL		0	NULL	NULL	NULL	gw70_nature_422_6929_302_s_138	12646920	To determine whether the internalization of NMDARs after glycine priming was mediated  through clathrin-dependent endocytosis, we made use of a dynamin inhibitory peptide,  QVPSRPNRAP, which competitively binds with the amphiphysin SH3 domain 15 and prevents endocytosis when administered intracellularly 5,  10.	transcription
54071	4	335124	7	NULL	NULL	0	NULL	dynamin inhibitory peptide			is					QVPSRPNRAP					NULL		0	NULL	NULL	NULL	gw70_nature_422_6929_302_s_138	12646920	To determine whether the internalization of NMDARs after glycine priming was mediated  through clathrin-dependent endocytosis, we made use of a dynamin inhibitory peptide,  QVPSRPNRAP, which competitively binds with the amphiphysin SH3 domain 15 and prevents endocytosis when administered intracellularly 5,  10.	transcription
53612	2	335126	5	NULL	NULL	0	NULL	Z1	NULL	mRNA splicing of	generates	NULL				statement 1	NULL				NULL		0	NULL	NULL	NULL	gw70_neuroscience_122_2_449_s_198	14614909	Of more interest is the fact that alternative mRNA splicing of  Z1 generates glycine  receptors that differ in their anatomical distribution;  Z1L transcript expression  is highly restricted to the rostral part of the telencephalon while  Z1 mRNA is expressed  all over the CNS ( Fig. 5).	transcription
53613	1	335126	5	NULL	NULL	0	NULL	glycine receptors	NULL		differ in	NULL				anatomical distribution	NULL				NULL		0	NULL	NULL	NULL	gw70_neuroscience_122_2_449_s_198	14614909	Of more interest is the fact that alternative mRNA splicing of  Z1 generates glycine  receptors that differ in their anatomical distribution;  Z1L transcript expression  is highly restricted to the rostral part of the telencephalon while  Z1 mRNA is expressed  all over the CNS ( Fig. 5).	transcription
53614	3	335126	5	NULL	NULL	0	NULL	Z1L transcript	NULL	expression of	is restricted to	NULL	highly			telencephalon	NULL	rostral part of			NULL		0	NULL	NULL	NULL	gw70_neuroscience_122_2_449_s_198	14614909	Of more interest is the fact that alternative mRNA splicing of  Z1 generates glycine  receptors that differ in their anatomical distribution;  Z1L transcript expression  is highly restricted to the rostral part of the telencephalon while  Z1 mRNA is expressed  all over the CNS ( Fig. 5).	transcription
53615	4	335126	5	NULL	NULL	0	NULL	Z1 mRNA	NULL		is expressed all over	NULL				CNS	NULL				NULL		0	NULL	NULL	NULL	gw70_neuroscience_122_2_449_s_198	14614909	Of more interest is the fact that alternative mRNA splicing of  Z1 generates glycine  receptors that differ in their anatomical distribution;  Z1L transcript expression  is highly restricted to the rostral part of the telencephalon while  Z1 mRNA is expressed  all over the CNS ( Fig. 5).	transcription
54072	1	335126	7	NULL	NULL	0	NULL	Z1		alternative mRNA splicing of	generates					glycine receptors					NULL		0	NULL	NULL	NULL	gw70_neuroscience_122_2_449_s_198	14614909	Of more interest is the fact that alternative mRNA splicing of  Z1 generates glycine  receptors that differ in their anatomical distribution;  Z1L transcript expression  is highly restricted to the rostral part of the telencephalon while  Z1 mRNA is expressed  all over the CNS ( Fig. 5).	transcription
54073	2	335126	7	NULL	NULL	0	NULL	Z1L transcript		expression of	is restricted to					 telencephalon		rostral part of			NULL		0	NULL	NULL	NULL	gw70_neuroscience_122_2_449_s_198	14614909	Of more interest is the fact that alternative mRNA splicing of  Z1 generates glycine  receptors that differ in their anatomical distribution;  Z1L transcript expression  is highly restricted to the rostral part of the telencephalon while  Z1 mRNA is expressed  all over the CNS ( Fig. 5).	transcription
54074	3	335126	7	NULL	NULL	0	NULL	Z1 mRNA			is expressed in					CNS		entire			NULL		NULL	NULL	NULL	NULL	gw70_neuroscience_122_2_449_s_198	14614909	Of more interest is the fact that alternative mRNA splicing of  Z1 generates glycine  receptors that differ in their anatomical distribution;  Z1L transcript expression  is highly restricted to the rostral part of the telencephalon while  Z1 mRNA is expressed  all over the CNS ( Fig. 5).	transcription
53616	1	335127	5	NULL	NULL	0	NULL	beta-TrCP	NULL		bind	NULL				mPER2	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_7_2795_s_335	15767683	Mutation of serine 477 and glycine 479 to alanine [mPER2(S477A/G479A)] abolished almost all detectable CKI -dependent beta-TrCP binding to mPER2 (Fig.  8B, lane 5), indicating that these residues function as a novel beta-TrCP binding motif.	transcription
53617	2	335127	5	NULL	NULL	0	NULL	statement 1	NULL		is dependent on	NULL				CKI	NULL				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_7_2795_s_335	15767683	Mutation of serine 477 and glycine 479 to alanine [mPER2(S477A/G479A)] abolished almost all detectable CKI -dependent beta-TrCP binding to mPER2 (Fig.  8B, lane 5), indicating that these residues function as a novel beta-TrCP binding motif.	transcription
53618	3	335127	5	NULL	NULL	0	NULL	mPER2	NULL	mutant	abolishes	NULL		(S477A/G479A)		statement 1	NULL				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_7_2795_s_335	15767683	Mutation of serine 477 and glycine 479 to alanine [mPER2(S477A/G479A)] abolished almost all detectable CKI -dependent beta-TrCP binding to mPER2 (Fig.  8B, lane 5), indicating that these residues function as a novel beta-TrCP binding motif.	transcription
53619	4	335127	5	NULL	NULL	0	NULL	mPER2	NULL		function as	NULL		S477		beta-TrCP binding motif	NULL	novel			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_7_2795_s_335	15767683	Mutation of serine 477 and glycine 479 to alanine [mPER2(S477A/G479A)] abolished almost all detectable CKI -dependent beta-TrCP binding to mPER2 (Fig.  8B, lane 5), indicating that these residues function as a novel beta-TrCP binding motif.	transcription
53620	5	335127	5	NULL	NULL	0	NULL	mPER2	NULL		function as	NULL		G479		beta-TrCP binding motif	NULL	novel			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_7_2795_s_335	15767683	Mutation of serine 477 and glycine 479 to alanine [mPER2(S477A/G479A)] abolished almost all detectable CKI -dependent beta-TrCP binding to mPER2 (Fig.  8B, lane 5), indicating that these residues function as a novel beta-TrCP binding motif.	transcription
54075	1	335127	7	NULL	NULL	0	NULL	beta-TrCP			bind					mPER2					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_7_2795_s_335	15767683	Mutation of serine 477 and glycine 479 to alanine [mPER2(S477A/G479A)] abolished almost all detectable CKI -dependent beta-TrCP binding to mPER2 (Fig.  8B, lane 5), indicating that these residues function as a novel beta-TrCP binding motif.	transcription
54076	2	335127	7	NULL	NULL	0	NULL	statement 1			depends on					CKI					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_7_2795_s_335	15767683	Mutation of serine 477 and glycine 479 to alanine [mPER2(S477A/G479A)] abolished almost all detectable CKI -dependent beta-TrCP binding to mPER2 (Fig.  8B, lane 5), indicating that these residues function as a novel beta-TrCP binding motif.	transcription
54077	3	335127	7	NULL	NULL	0	NULL	mPER2		mutant	abolish			S477A		statement 1					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_7_2795_s_335	15767683	Mutation of serine 477 and glycine 479 to alanine [mPER2(S477A/G479A)] abolished almost all detectable CKI -dependent beta-TrCP binding to mPER2 (Fig.  8B, lane 5), indicating that these residues function as a novel beta-TrCP binding motif.	transcription
54078	4	335127	7	NULL	NULL	0	NULL	mPER2		mutant	abolish			G479A		statement 1					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_7_2795_s_335	15767683	Mutation of serine 477 and glycine 479 to alanine [mPER2(S477A/G479A)] abolished almost all detectable CKI -dependent beta-TrCP binding to mPER2 (Fig.  8B, lane 5), indicating that these residues function as a novel beta-TrCP binding motif.	transcription
54079	5	335127	7	NULL	NULL	0	NULL	mPER2			function as			serine 477		mPER2			novel beta-TrCP binding motif		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_7_2795_s_335	15767683	Mutation of serine 477 and glycine 479 to alanine [mPER2(S477A/G479A)] abolished almost all detectable CKI -dependent beta-TrCP binding to mPER2 (Fig.  8B, lane 5), indicating that these residues function as a novel beta-TrCP binding motif.	transcription
54080	6	335127	7	NULL	NULL	0	NULL	mPER2			function as			glycine 479		mPER2			novel beta-TrCP binding motif		NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_7_2795_s_335	15767683	Mutation of serine 477 and glycine 479 to alanine [mPER2(S477A/G479A)] abolished almost all detectable CKI -dependent beta-TrCP binding to mPER2 (Fig.  8B, lane 5), indicating that these residues function as a novel beta-TrCP binding motif.	transcription
53621	1	335128	5	NULL	NULL	0	NULL	insulin-like growth factor-binding protein 5	NULL	rat	is mutated to	NULL		glycine		insulin-like growth factor-binding protein 5	NULL	rat	glutamine		NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_9_2841_s_312	15090526	Another study, involving a mutation in rat insulin-like growth factor-binding protein 5, has also shown that replacement of a critical glycine with glutamine causes the protein to lose activity, although the mutation did not result in gross conformational changes in the protein ( ).	transcription
53622	2	335128	5	NULL	NULL	0	NULL	statement 1	NULL		causes	NULL				insulin-like growth factor-binding protein 5	NULL	loss of activity of;;rat			NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_9_2841_s_312	15090526	Another study, involving a mutation in rat insulin-like growth factor-binding protein 5, has also shown that replacement of a critical glycine with glutamine causes the protein to lose activity, although the mutation did not result in gross conformational changes in the protein ( ).	transcription
53623	3	335128	5	NULL	NULL	0	NULL	statement 1	NULL		does not result in	NULL				insulin-like growth factor-binding protein 5	NULL	gross conformational change of;;rat			NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_9_2841_s_312	15090526	Another study, involving a mutation in rat insulin-like growth factor-binding protein 5, has also shown that replacement of a critical glycine with glutamine causes the protein to lose activity, although the mutation did not result in gross conformational changes in the protein ( ).	transcription
54081	1	335128	7	NULL	NULL	0	NULL	insulin-like growth factor-binding protein 5		rat	is mutated to			glycine		insulin-like growth factor-binding protein 5		rat	glutamine		NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_9_2841_s_312	15090526	Another study, involving a mutation in rat insulin-like growth factor-binding protein 5, has also shown that replacement of a critical glycine with glutamine causes the protein to lose activity, although the mutation did not result in gross conformational changes in the protein ( ).	transcription
54082	2	335128	7	NULL	NULL	0	NULL	statement 1			cause					protein		loss of;; activity of			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_9_2841_s_312	15090526	Another study, involving a mutation in rat insulin-like growth factor-binding protein 5, has also shown that replacement of a critical glycine with glutamine causes the protein to lose activity, although the mutation did not result in gross conformational changes in the protein ( ).	transcription
54083	3	335128	7	NULL	NULL	0	NULL	statement 1			does not result in					protein		gross conformational changes in			NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_9_2841_s_312	15090526	Another study, involving a mutation in rat insulin-like growth factor-binding protein 5, has also shown that replacement of a critical glycine with glutamine causes the protein to lose activity, although the mutation did not result in gross conformational changes in the protein ( ).	transcription
53624	1	335129	5	NULL	NULL	0	NULL	phage A1-9	NULL		bind	NULL				OppA-1	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_1_51_s_175	14679224	To investigate whether changes in pH affect the affinity of OppA for its peptide substrates, phage A1-9, which binds to both OppA-1 and OppA-3, was diluted to the final concentration of 109 PFU in different pH buffers (0.2 M glycine-HCl for pHs 2.2 and 3; 100 mM Tris-HCl for pHs 5, 6, 7.	transcription
53625	2	335129	5	NULL	NULL	0	NULL	phage A1-9	NULL		bind	NULL				OppA-3	NULL				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_1_51_s_175	14679224	To investigate whether changes in pH affect the affinity of OppA for its peptide substrates, phage A1-9, which binds to both OppA-1 and OppA-3, was diluted to the final concentration of 109 PFU in different pH buffers (0.2 M glycine-HCl for pHs 2.2 and 3; 100 mM Tris-HCl for pHs 5, 6, 7.	transcription
54084	1	335129	7	NULL	NULL	0	NULL	OppA			has affinity for					peptide substrates					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_1_51_s_175	14679224	To investigate whether changes in pH affect the affinity of OppA for its peptide substrates, phage A1-9, which binds to both OppA-1 and OppA-3, was diluted to the final concentration of 109 PFU in different pH buffers (0.2 M glycine-HCl for pHs 2.2 and 3; 100 mM Tris-HCl for pHs 5, 6, 7.	transcription
54085	2	335129	7	NULL	NULL	0	NULL	phage A1-9			bind					OppA-1					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_1_51_s_175	14679224	To investigate whether changes in pH affect the affinity of OppA for its peptide substrates, phage A1-9, which binds to both OppA-1 and OppA-3, was diluted to the final concentration of 109 PFU in different pH buffers (0.2 M glycine-HCl for pHs 2.2 and 3; 100 mM Tris-HCl for pHs 5, 6, 7.	transcription
54086	3	335129	7	NULL	NULL	0	NULL	phage A1-9			bind					OppA-3					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_1_51_s_175	14679224	To investigate whether changes in pH affect the affinity of OppA for its peptide substrates, phage A1-9, which binds to both OppA-1 and OppA-3, was diluted to the final concentration of 109 PFU in different pH buffers (0.2 M glycine-HCl for pHs 2.2 and 3; 100 mM Tris-HCl for pHs 5, 6, 7.	transcription
53626	1	335130	5	NULL	NULL	0	NULL	PMTS	NULL		enhances	NULL				GlyR	NULL	function of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_6_3305_s_66	16361257	However, before using this approach to examine binding pocket occupancy, we showed that 5 mM PMTS enhances GlyR function like alcohols or anesthetics when directly co-applied to wt and S267C GlyRs with an EC10 concentration of glycine ( Fig. 2).	transcription
54763	1	335130	7	NULL	NULL	0	NULL	PMTS			enhance					GlyR		function of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_6_3305_s_66	16361257	However, before using this approach to examine binding pocket occupancy, we showed that 5 mM PMTS enhances GlyR function like alcohols or anesthetics when directly co-applied to wt and S267C GlyRs with an EC10 concentration of glycine ( Fig. 2).	transcription
54764	2	335130	7	NULL	NULL	0	NULL	alcohols			enhance					GlyR		function of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_6_3305_s_66	16361257	However, before using this approach to examine binding pocket occupancy, we showed that 5 mM PMTS enhances GlyR function like alcohols or anesthetics when directly co-applied to wt and S267C GlyRs with an EC10 concentration of glycine ( Fig. 2).	transcription
54765	3	335130	7	NULL	NULL	0	NULL	anesthetics			enhance					GlyR		function of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_6_3305_s_66	16361257	However, before using this approach to examine binding pocket occupancy, we showed that 5 mM PMTS enhances GlyR function like alcohols or anesthetics when directly co-applied to wt and S267C GlyRs with an EC10 concentration of glycine ( Fig. 2).	transcription
54766	4	335130	7	NULL	NULL	0	NULL	statement 2			is an alternative to					statement 3					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_6_3305_s_66	16361257	However, before using this approach to examine binding pocket occupancy, we showed that 5 mM PMTS enhances GlyR function like alcohols or anesthetics when directly co-applied to wt and S267C GlyRs with an EC10 concentration of glycine ( Fig. 2).	transcription
53665	1	335132	5	NULL	NULL	0	NULL	amino acid		specific composition of	plays a role in		central					binding of	ALE-1-targeting domain		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_549_s_261	16257954	Evidently, the specific amino acid composition and the length of the interpeptide bridge play central roles in ALE-1-targeting domain binding; substitution of glycine by serine at position 3 or 5 significantly impairs the gross binding of the targeting domain to staphylococcal PGs, while the length of the interpeptide bridges,  i.e. pentaglycine, confers the maximum binding of the targeting domain to PGs.	transcription
53666	2	335132	5	NULL	NULL	0	NULL	interpeptide bridge		length of	plays a role in		central					binding of	ALE-1-targeting domain		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_549_s_261	16257954	Evidently, the specific amino acid composition and the length of the interpeptide bridge play central roles in ALE-1-targeting domain binding; substitution of glycine by serine at position 3 or 5 significantly impairs the gross binding of the targeting domain to staphylococcal PGs, while the length of the interpeptide bridges,  i.e. pentaglycine, confers the maximum binding of the targeting domain to PGs.	transcription
53667	3	335132	5	NULL	NULL	0	NULL				bind			targeting domain		PGs		staphylococcal			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_549_s_261	16257954	Evidently, the specific amino acid composition and the length of the interpeptide bridge play central roles in ALE-1-targeting domain binding; substitution of glycine by serine at position 3 or 5 significantly impairs the gross binding of the targeting domain to staphylococcal PGs, while the length of the interpeptide bridges,  i.e. pentaglycine, confers the maximum binding of the targeting domain to PGs.	transcription
53668	4	335132	5	NULL	NULL	0	NULL	glycine			is substituted to			position 3		serine					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_1_549_s_261	16257954	Evidently, the specific amino acid composition and the length of the interpeptide bridge play central roles in ALE-1-targeting domain binding; substitution of glycine by serine at position 3 or 5 significantly impairs the gross binding of the targeting domain to staphylococcal PGs, while the length of the interpeptide bridges,  i.e. pentaglycine, confers the maximum binding of the targeting domain to PGs.	transcription
53669	5	335132	5	NULL	NULL	0	NULL	glycine			is substituted to			position 5		serine					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_549_s_261	16257954	Evidently, the specific amino acid composition and the length of the interpeptide bridge play central roles in ALE-1-targeting domain binding; substitution of glycine by serine at position 3 or 5 significantly impairs the gross binding of the targeting domain to staphylococcal PGs, while the length of the interpeptide bridges,  i.e. pentaglycine, confers the maximum binding of the targeting domain to PGs.	transcription
53670	6	335132	5	NULL	NULL	0	NULL	statement 4			impairs					statement 3					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_549_s_261	16257954	Evidently, the specific amino acid composition and the length of the interpeptide bridge play central roles in ALE-1-targeting domain binding; substitution of glycine by serine at position 3 or 5 significantly impairs the gross binding of the targeting domain to staphylococcal PGs, while the length of the interpeptide bridges,  i.e. pentaglycine, confers the maximum binding of the targeting domain to PGs.	transcription
53671	7	335132	5	NULL	NULL	0	NULL	statement 5			impairs					statement 3					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_549_s_261	16257954	Evidently, the specific amino acid composition and the length of the interpeptide bridge play central roles in ALE-1-targeting domain binding; substitution of glycine by serine at position 3 or 5 significantly impairs the gross binding of the targeting domain to staphylococcal PGs, while the length of the interpeptide bridges,  i.e. pentaglycine, confers the maximum binding of the targeting domain to PGs.	transcription
53672	8	335132	5	NULL	NULL	0	NULL	pentaglycine			confers					statement 3		maximum binding of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_549_s_261	16257954	Evidently, the specific amino acid composition and the length of the interpeptide bridge play central roles in ALE-1-targeting domain binding; substitution of glycine by serine at position 3 or 5 significantly impairs the gross binding of the targeting domain to staphylococcal PGs, while the length of the interpeptide bridges,  i.e. pentaglycine, confers the maximum binding of the targeting domain to PGs.	transcription
54767	1	335132	7	NULL	NULL	0	NULL				bind			ALE-1-targeting domain		PGs				staphylococcal	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_549_s_261	16257954	Evidently, the specific amino acid composition and the length of the interpeptide bridge play central roles in ALE-1-targeting domain binding; substitution of glycine by serine at position 3 or 5 significantly impairs the gross binding of the targeting domain to staphylococcal PGs, while the length of the interpeptide bridges,  i.e. pentaglycine, confers the maximum binding of the targeting domain to PGs.	transcription
54768	2	335132	7	NULL	NULL	0	NULL				substituted for			ALE-1-targeting domain;;glycine 3					ALE-1-targeting domain;;serine 3		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_549_s_261	16257954	Evidently, the specific amino acid composition and the length of the interpeptide bridge play central roles in ALE-1-targeting domain binding; substitution of glycine by serine at position 3 or 5 significantly impairs the gross binding of the targeting domain to staphylococcal PGs, while the length of the interpeptide bridges,  i.e. pentaglycine, confers the maximum binding of the targeting domain to PGs.	transcription
54769	3	335132	7	NULL	NULL	0	NULL				substituted for			ALE-1-targeting domain;;glycine 5					ALE-1-targeting domain;;serine 5		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_549_s_261	16257954	Evidently, the specific amino acid composition and the length of the interpeptide bridge play central roles in ALE-1-targeting domain binding; substitution of glycine by serine at position 3 or 5 significantly impairs the gross binding of the targeting domain to staphylococcal PGs, while the length of the interpeptide bridges,  i.e. pentaglycine, confers the maximum binding of the targeting domain to PGs.	transcription
54770	4	335132	7	NULL	NULL	0	NULL	statement 2			impairs		significantly			statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_549_s_261	16257954	Evidently, the specific amino acid composition and the length of the interpeptide bridge play central roles in ALE-1-targeting domain binding; substitution of glycine by serine at position 3 or 5 significantly impairs the gross binding of the targeting domain to staphylococcal PGs, while the length of the interpeptide bridges,  i.e. pentaglycine, confers the maximum binding of the targeting domain to PGs.	transcription
54771	5	335132	7	NULL	NULL	0	NULL	statement 3			impairs		significantly			statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_549_s_261	16257954	Evidently, the specific amino acid composition and the length of the interpeptide bridge play central roles in ALE-1-targeting domain binding; substitution of glycine by serine at position 3 or 5 significantly impairs the gross binding of the targeting domain to staphylococcal PGs, while the length of the interpeptide bridges,  i.e. pentaglycine, confers the maximum binding of the targeting domain to PGs.	transcription
54772	6	335132	7	NULL	NULL	0	NULL	pentaglycine		interpeptide bridge of	confers					statement 1		maximum binding of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_1_549_s_261	16257954	Evidently, the specific amino acid composition and the length of the interpeptide bridge play central roles in ALE-1-targeting domain binding; substitution of glycine by serine at position 3 or 5 significantly impairs the gross binding of the targeting domain to staphylococcal PGs, while the length of the interpeptide bridges,  i.e. pentaglycine, confers the maximum binding of the targeting domain to PGs.	transcription
53673	1	335133	5	NULL	NULL	0	NULL	NMDA			induce					[Ca2+]i		increase in			NULL		0	NULL	NULL	NULL	gw70_jneurosci_26_13_3404_s_85	16571747	E, Administration of 500 muM NMDA (in Mg2+-free KRH, containing 5 muM glycine) induces both a [Ca2+]i increase and a PKCgamma-EGFP translocation that are completely reverted by a NMDAR blocker (100 muM APV, in the presence of 1.2 mM Mg2+).	transcription
53674	2	335133	5	NULL	NULL	0	NULL	NMDA			induce					PKCgamma-EGFP		translocation of			NULL		0	NULL	NULL	NULL	gw70_jneurosci_26_13_3404_s_85	16571747	E, Administration of 500 muM NMDA (in Mg2+-free KRH, containing 5 muM glycine) induces both a [Ca2+]i increase and a PKCgamma-EGFP translocation that are completely reverted by a NMDAR blocker (100 muM APV, in the presence of 1.2 mM Mg2+).	transcription
53675	3	335133	5	NULL	NULL	0	NULL	NMDAR blocker			reverts		completely			statement 1					NULL		0	NULL	NULL	NULL	gw70_jneurosci_26_13_3404_s_85	16571747	E, Administration of 500 muM NMDA (in Mg2+-free KRH, containing 5 muM glycine) induces both a [Ca2+]i increase and a PKCgamma-EGFP translocation that are completely reverted by a NMDAR blocker (100 muM APV, in the presence of 1.2 mM Mg2+).	transcription
53676	4	335133	5	NULL	NULL	0	NULL	NMDAR blocker			reverts		completely			statement 2					NULL		0	NULL	NULL	NULL	gw70_jneurosci_26_13_3404_s_85	16571747	E, Administration of 500 muM NMDA (in Mg2+-free KRH, containing 5 muM glycine) induces both a [Ca2+]i increase and a PKCgamma-EGFP translocation that are completely reverted by a NMDAR blocker (100 muM APV, in the presence of 1.2 mM Mg2+).	transcription
54773	1	335133	7	NULL	NULL	0	NULL	 PKCgamma			translocates					EGFP					NULL		0	NULL	NULL	NULL	gw70_jneurosci_26_13_3404_s_85	16571747	E, Administration of 500 muM NMDA (in Mg2+-free KRH, containing 5 muM glycine) induces both a [Ca2+]i increase and a PKCgamma-EGFP translocation that are completely reverted by a NMDAR blocker (100 muM APV, in the presence of 1.2 mM Mg2+).	transcription
54774	2	335133	7	NULL	NULL	0	NULL	NMDA 			induce					[Ca2+]i		increase of			NULL		0	NULL	NULL	NULL	gw70_jneurosci_26_13_3404_s_85	16571747	E, Administration of 500 muM NMDA (in Mg2+-free KRH, containing 5 muM glycine) induces both a [Ca2+]i increase and a PKCgamma-EGFP translocation that are completely reverted by a NMDAR blocker (100 muM APV, in the presence of 1.2 mM Mg2+).	transcription
54775	3	335133	7	NULL	NULL	0	NULL	NMDA			induce					statement 1					NULL		0	NULL	NULL	NULL	gw70_jneurosci_26_13_3404_s_85	16571747	E, Administration of 500 muM NMDA (in Mg2+-free KRH, containing 5 muM glycine) induces both a [Ca2+]i increase and a PKCgamma-EGFP translocation that are completely reverted by a NMDAR blocker (100 muM APV, in the presence of 1.2 mM Mg2+).	transcription
54776	4	335133	7	NULL	NULL	0	NULL	NMDAR blocker			reverts		completely			statement 2					NULL		0	NULL	NULL	NULL	gw70_jneurosci_26_13_3404_s_85	16571747	E, Administration of 500 muM NMDA (in Mg2+-free KRH, containing 5 muM glycine) induces both a [Ca2+]i increase and a PKCgamma-EGFP translocation that are completely reverted by a NMDAR blocker (100 muM APV, in the presence of 1.2 mM Mg2+).	transcription
54777	5	335133	7	NULL	NULL	0	NULL	NMDAR blocker			reverts		completely			statement 4					NULL		NULL	NULL	NULL	NULL	gw70_jneurosci_26_13_3404_s_85	16571747	E, Administration of 500 muM NMDA (in Mg2+-free KRH, containing 5 muM glycine) induces both a [Ca2+]i increase and a PKCgamma-EGFP translocation that are completely reverted by a NMDAR blocker (100 muM APV, in the presence of 1.2 mM Mg2+).	transcription
54822	1	335134	7	NULL	NULL	0	NULL	HF-Cui1 			bind					Cdc48 proteins					NULL		0	NULL	NULL	NULL	gw70_yeast_21_2_127_s_76	14755638	The column was then washed with 3 x 5 ml TBS buffer (150 mM NaCl, 50 mM Tris-HCl, pH 7.5) and the bound HF-Cui1 and Cdc48 proteins eluted using 3 x 0.25  ml of 0.1 M glycine, pH 3.5.	transcription
53677	1	335135	5	NULL	NULL	0	NULL	RPS19 protein		mature	replaces		functionally;;possibly	RNA-binding portion		ribosomal protein					NULL		NULL	NULL	NULL	NULL	gw60_genetics_158_3_1289_s_214	11454775	Most of the RNA-binding protein, minus the glycine-rich C terminus, is found at the 5' end of  rps19, and the RNA-binding portion of the mature RPS19 protein has been proposed to functionally replace another ribosomal protein ( S ANCHEZ et al. 1996   ).	transcription
56140	1	335135	7	NULL	NULL	0	NULL	RNA-binding protein			bind					rps19			 5' end of		NULL		0	NULL	NULL	NULL	gw60_genetics_158_3_1289_s_214	11454775	Most of the RNA-binding protein, minus the glycine-rich C terminus, is found at the 5' end of  rps19, and the RNA-binding portion of the mature RPS19 protein has been proposed to functionally replace another ribosomal protein ( S ANCHEZ et al. 1996   ).	transcription
53678	1	335138	5	NULL	NULL	0	NULL	NMDA			induce					seizures					NULL	mice	0	NULL	NULL	NULL	gw60_brainres_944_1_165_s_172	12106676	Comparison of the anticonvulsant activities of NMDA receptor glycine-binding site antagonists on NMDA-induced seizures in mice      (<1K) Drugs were administered intravenously via the tail vein 20 min before intracerebroventricular injection of NMDA (5 nmol/10  l per mouse).	transcription
54823	1	335138	7	NULL	NULL	0	NULL	NMDA			induce					seizure					NULL	mice	0	NULL	NULL	NULL	gw60_brainres_944_1_165_s_172	12106676	Comparison of the anticonvulsant activities of NMDA receptor glycine-binding site antagonists on NMDA-induced seizures in mice      (<1K) Drugs were administered intravenously via the tail vein 20 min before intracerebroventricular injection of NMDA (5 nmol/10  l per mouse).	transcription
53679	1	335140	5	NULL	NULL	0	NULL	chlormethiazole			does not affect					glycine responses					NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_126_3_801_s_160	10188994	The inability of chlormethiazole to affect glycine responses (on either side of ECl) was confirmed by using a higher concentration (100 muM) in seven additional cells, continuously perfused with bicuculline (5 muM) in order to block GABA responses and to prevent the leak current increase usually induced by chlormethiazole ( Figure 5f).	transcription
54824	1	335140	7	NULL	NULL	0	NULL	chlormethiazole			does not affect					glycine		response of			NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_126_3_801_s_160	10188994	The inability of chlormethiazole to affect glycine responses (on either side of ECl) was confirmed by using a higher concentration (100 muM) in seven additional cells, continuously perfused with bicuculline (5 muM) in order to block GABA responses and to prevent the leak current increase usually induced by chlormethiazole ( Figure 5f).	transcription
54825	2	335140	7	NULL	NULL	0	NULL	bicuculline			block					GABA 		response of			NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_126_3_801_s_160	10188994	The inability of chlormethiazole to affect glycine responses (on either side of ECl) was confirmed by using a higher concentration (100 muM) in seven additional cells, continuously perfused with bicuculline (5 muM) in order to block GABA responses and to prevent the leak current increase usually induced by chlormethiazole ( Figure 5f).	transcription
53680	1	335143	5	NULL	NULL	0	NULL	LDL			is mutated to			Asp235		LDL			glycine		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1392_s_160	9261272	2  Interestingly, another point mutation in the same codon as FH-Keuruu, changing aspartic acid to the neutral amino acid glycine (Asp235 Gly or FH Nevers), was found to result in an LDL receptor with only 5% to 15% of activity compared to the normal one.	transcription
53681	2	335143	5	NULL	NULL	0	NULL			point mutation of	leads to			FH-Keuruu		statement 1					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1392_s_160	9261272	2  Interestingly, another point mutation in the same codon as FH-Keuruu, changing aspartic acid to the neutral amino acid glycine (Asp235 Gly or FH Nevers), was found to result in an LDL receptor with only 5% to 15% of activity compared to the normal one.	transcription
53682	3	335143	5	NULL	NULL	0	NULL	statement 1		activity of	lesser than					LDL		normal			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1392_s_160	9261272	2  Interestingly, another point mutation in the same codon as FH-Keuruu, changing aspartic acid to the neutral amino acid glycine (Asp235 Gly or FH Nevers), was found to result in an LDL receptor with only 5% to 15% of activity compared to the normal one.	transcription
53683	4	335143	5	NULL	NULL	0	NULL	glycine			is a type of					neutral amino acid					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1392_s_160	9261272	2  Interestingly, another point mutation in the same codon as FH-Keuruu, changing aspartic acid to the neutral amino acid glycine (Asp235 Gly or FH Nevers), was found to result in an LDL receptor with only 5% to 15% of activity compared to the normal one.	transcription
56141	1	335143	7	NULL	NULL	0	NULL	LDL			is mutated to			Asp235 		LDL			glycine		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1392_s_160	9261272	2  Interestingly, another point mutation in the same codon as FH-Keuruu, changing aspartic acid to the neutral amino acid glycine (Asp235 Gly or FH Nevers), was found to result in an LDL receptor with only 5% to 15% of activity compared to the normal one.	transcription
56142	2	335143	7	NULL	NULL	0	NULL	FH-Keuruu		 point mutation of	leads to 					statement 1					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1392_s_160	9261272	2  Interestingly, another point mutation in the same codon as FH-Keuruu, changing aspartic acid to the neutral amino acid glycine (Asp235 Gly or FH Nevers), was found to result in an LDL receptor with only 5% to 15% of activity compared to the normal one.	transcription
56143	3	335143	7	NULL	NULL	0	NULL	statement 1		activity of	is lesser than					LDL		normal			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1392_s_160	9261272	2  Interestingly, another point mutation in the same codon as FH-Keuruu, changing aspartic acid to the neutral amino acid glycine (Asp235 Gly or FH Nevers), was found to result in an LDL receptor with only 5% to 15% of activity compared to the normal one.	transcription
56144	4	335143	7	NULL	NULL	0	NULL	glycine			is a type of					neutral amino acid					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_17_7_1392_s_160	9261272	2  Interestingly, another point mutation in the same codon as FH-Keuruu, changing aspartic acid to the neutral amino acid glycine (Asp235 Gly or FH Nevers), was found to result in an LDL receptor with only 5% to 15% of activity compared to the normal one.	transcription
53684	1	335145	5	NULL	NULL	0	NULL	bicuculline			is an antagonist of					GABAA receptor					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_39_12_2231_s_54	10974307	Bath application of the GABAA receptor antagonists bicuculline or picrotoxin and the glycine receptor antagonist strychnine typically increased the duration of EPSPs and EPSCs and the cell excitability but had little or no effect on the amplitude and slope of the initial component of both responses (see the traces in  Fig. 3,  Fig. 4 and  Fig. 5).	transcription
53685	2	335145	5	NULL	NULL	0	NULL	picrotoxin			is an antagonist of					GABAA receptor					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_39_12_2231_s_54	10974307	Bath application of the GABAA receptor antagonists bicuculline or picrotoxin and the glycine receptor antagonist strychnine typically increased the duration of EPSPs and EPSCs and the cell excitability but had little or no effect on the amplitude and slope of the initial component of both responses (see the traces in  Fig. 3,  Fig. 4 and  Fig. 5).	transcription
53686	3	335145	5	NULL	NULL	0	NULL	strychnine			is an antagonist of					glycine receptor					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_39_12_2231_s_54	10974307	Bath application of the GABAA receptor antagonists bicuculline or picrotoxin and the glycine receptor antagonist strychnine typically increased the duration of EPSPs and EPSCs and the cell excitability but had little or no effect on the amplitude and slope of the initial component of both responses (see the traces in  Fig. 3,  Fig. 4 and  Fig. 5).	transcription
53687	4	335145	5	NULL	NULL	0	NULL	bicuculline			increases					EPSPs		duration of			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_39_12_2231_s_54	10974307	Bath application of the GABAA receptor antagonists bicuculline or picrotoxin and the glycine receptor antagonist strychnine typically increased the duration of EPSPs and EPSCs and the cell excitability but had little or no effect on the amplitude and slope of the initial component of both responses (see the traces in  Fig. 3,  Fig. 4 and  Fig. 5).	transcription
53688	5	335145	5	NULL	NULL	0	NULL	picrotoxin			increases					EPSPs		duration of			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_39_12_2231_s_54	10974307	Bath application of the GABAA receptor antagonists bicuculline or picrotoxin and the glycine receptor antagonist strychnine typically increased the duration of EPSPs and EPSCs and the cell excitability but had little or no effect on the amplitude and slope of the initial component of both responses (see the traces in  Fig. 3,  Fig. 4 and  Fig. 5).	transcription
53689	6	335145	5	NULL	NULL	0	NULL	strychnine			increases					EPSPs		duration of			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_39_12_2231_s_54	10974307	Bath application of the GABAA receptor antagonists bicuculline or picrotoxin and the glycine receptor antagonist strychnine typically increased the duration of EPSPs and EPSCs and the cell excitability but had little or no effect on the amplitude and slope of the initial component of both responses (see the traces in  Fig. 3,  Fig. 4 and  Fig. 5).	transcription
53690	7	335145	5	NULL	NULL	0	NULL	bicuculline			increases					EPSCs		duration of			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_39_12_2231_s_54	10974307	Bath application of the GABAA receptor antagonists bicuculline or picrotoxin and the glycine receptor antagonist strychnine typically increased the duration of EPSPs and EPSCs and the cell excitability but had little or no effect on the amplitude and slope of the initial component of both responses (see the traces in  Fig. 3,  Fig. 4 and  Fig. 5).	transcription
53691	8	335145	5	NULL	NULL	0	NULL	picrotoxin			increases					EPSCs		duration of			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_39_12_2231_s_54	10974307	Bath application of the GABAA receptor antagonists bicuculline or picrotoxin and the glycine receptor antagonist strychnine typically increased the duration of EPSPs and EPSCs and the cell excitability but had little or no effect on the amplitude and slope of the initial component of both responses (see the traces in  Fig. 3,  Fig. 4 and  Fig. 5).	transcription
53692	9	335145	5	NULL	NULL	0	NULL	strychnine			increases					EPSCs		duration of			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_39_12_2231_s_54	10974307	Bath application of the GABAA receptor antagonists bicuculline or picrotoxin and the glycine receptor antagonist strychnine typically increased the duration of EPSPs and EPSCs and the cell excitability but had little or no effect on the amplitude and slope of the initial component of both responses (see the traces in  Fig. 3,  Fig. 4 and  Fig. 5).	transcription
53693	10	335145	5	NULL	NULL	0	NULL	bicuculline			increases					cell		excitability of			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_39_12_2231_s_54	10974307	Bath application of the GABAA receptor antagonists bicuculline or picrotoxin and the glycine receptor antagonist strychnine typically increased the duration of EPSPs and EPSCs and the cell excitability but had little or no effect on the amplitude and slope of the initial component of both responses (see the traces in  Fig. 3,  Fig. 4 and  Fig. 5).	transcription
53694	11	335145	5	NULL	NULL	0	NULL	picrotoxin			increases					cell		excitability of			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_39_12_2231_s_54	10974307	Bath application of the GABAA receptor antagonists bicuculline or picrotoxin and the glycine receptor antagonist strychnine typically increased the duration of EPSPs and EPSCs and the cell excitability but had little or no effect on the amplitude and slope of the initial component of both responses (see the traces in  Fig. 3,  Fig. 4 and  Fig. 5).	transcription
53695	12	335145	5	NULL	NULL	0	NULL	strychnine			increases					cell		excitability of			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_39_12_2231_s_54	10974307	Bath application of the GABAA receptor antagonists bicuculline or picrotoxin and the glycine receptor antagonist strychnine typically increased the duration of EPSPs and EPSCs and the cell excitability but had little or no effect on the amplitude and slope of the initial component of both responses (see the traces in  Fig. 3,  Fig. 4 and  Fig. 5).	transcription
54837	1	335145	7	NULL	NULL	0	NULL	bicuculline 			increase 					EPSPs		duration of			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_39_12_2231_s_54	10974307	Bath application of the GABAA receptor antagonists bicuculline or picrotoxin and the glycine receptor antagonist strychnine typically increased the duration of EPSPs and EPSCs and the cell excitability but had little or no effect on the amplitude and slope of the initial component of both responses (see the traces in  Fig. 3,  Fig. 4 and  Fig. 5).	transcription
54838	2	335145	7	NULL	NULL	0	NULL	bicuculline			increase					EPSCs		duration of			NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_39_12_2231_s_54	10974307	Bath application of the GABAA receptor antagonists bicuculline or picrotoxin and the glycine receptor antagonist strychnine typically increased the duration of EPSPs and EPSCs and the cell excitability but had little or no effect on the amplitude and slope of the initial component of both responses (see the traces in  Fig. 3,  Fig. 4 and  Fig. 5).	transcription
54839	3	335145	7	NULL	NULL	0	NULL	 bicuculline			increase					cell excitability		duration of			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_39_12_2231_s_54	10974307	Bath application of the GABAA receptor antagonists bicuculline or picrotoxin and the glycine receptor antagonist strychnine typically increased the duration of EPSPs and EPSCs and the cell excitability but had little or no effect on the amplitude and slope of the initial component of both responses (see the traces in  Fig. 3,  Fig. 4 and  Fig. 5).	transcription
54840	4	335145	7	NULL	NULL	0	NULL	picrotoxin			increase					EPSPs		duration of			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_39_12_2231_s_54	10974307	Bath application of the GABAA receptor antagonists bicuculline or picrotoxin and the glycine receptor antagonist strychnine typically increased the duration of EPSPs and EPSCs and the cell excitability but had little or no effect on the amplitude and slope of the initial component of both responses (see the traces in  Fig. 3,  Fig. 4 and  Fig. 5).	transcription
54841	5	335145	7	NULL	NULL	0	NULL	picrotoxin			increase					EPSCs		duration of			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_39_12_2231_s_54	10974307	Bath application of the GABAA receptor antagonists bicuculline or picrotoxin and the glycine receptor antagonist strychnine typically increased the duration of EPSPs and EPSCs and the cell excitability but had little or no effect on the amplitude and slope of the initial component of both responses (see the traces in  Fig. 3,  Fig. 4 and  Fig. 5).	transcription
54842	6	335145	7	NULL	NULL	0	NULL	picrotoxin			increase					cell excitability		duration of			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_39_12_2231_s_54	10974307	Bath application of the GABAA receptor antagonists bicuculline or picrotoxin and the glycine receptor antagonist strychnine typically increased the duration of EPSPs and EPSCs and the cell excitability but had little or no effect on the amplitude and slope of the initial component of both responses (see the traces in  Fig. 3,  Fig. 4 and  Fig. 5).	transcription
54843	7	335145	7	NULL	NULL	0	NULL	strychnine			increase					EPSPs		duration of			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_39_12_2231_s_54	10974307	Bath application of the GABAA receptor antagonists bicuculline or picrotoxin and the glycine receptor antagonist strychnine typically increased the duration of EPSPs and EPSCs and the cell excitability but had little or no effect on the amplitude and slope of the initial component of both responses (see the traces in  Fig. 3,  Fig. 4 and  Fig. 5).	transcription
54844	8	335145	7	NULL	NULL	0	NULL	strychnine			increase					EPSCs		duration of			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_39_12_2231_s_54	10974307	Bath application of the GABAA receptor antagonists bicuculline or picrotoxin and the glycine receptor antagonist strychnine typically increased the duration of EPSPs and EPSCs and the cell excitability but had little or no effect on the amplitude and slope of the initial component of both responses (see the traces in  Fig. 3,  Fig. 4 and  Fig. 5).	transcription
55136	9	335145	7	NULL	NULL	0	NULL	strychnine			increase					cell excitability		duration of			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_39_12_2231_s_54	10974307	Bath application of the GABAA receptor antagonists bicuculline or picrotoxin and the glycine receptor antagonist strychnine typically increased the duration of EPSPs and EPSCs and the cell excitability but had little or no effect on the amplitude and slope of the initial component of both responses (see the traces in  Fig. 3,  Fig. 4 and  Fig. 5).	transcription
55137	10	335145	7	NULL	NULL	0	NULL	bicuculline			is a type of					GABAA receptor antagonist					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_39_12_2231_s_54	10974307	Bath application of the GABAA receptor antagonists bicuculline or picrotoxin and the glycine receptor antagonist strychnine typically increased the duration of EPSPs and EPSCs and the cell excitability but had little or no effect on the amplitude and slope of the initial component of both responses (see the traces in  Fig. 3,  Fig. 4 and  Fig. 5).	transcription
55138	11	335145	7	NULL	NULL	0	NULL	picrotoxin			is a type of					GABAA receptor antagonist					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_39_12_2231_s_54	10974307	Bath application of the GABAA receptor antagonists bicuculline or picrotoxin and the glycine receptor antagonist strychnine typically increased the duration of EPSPs and EPSCs and the cell excitability but had little or no effect on the amplitude and slope of the initial component of both responses (see the traces in  Fig. 3,  Fig. 4 and  Fig. 5).	transcription
55139	12	335145	7	NULL	NULL	0	NULL	strychnine			is a type of					 glycine receptor antagonist					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_39_12_2231_s_54	10974307	Bath application of the GABAA receptor antagonists bicuculline or picrotoxin and the glycine receptor antagonist strychnine typically increased the duration of EPSPs and EPSCs and the cell excitability but had little or no effect on the amplitude and slope of the initial component of both responses (see the traces in  Fig. 3,  Fig. 4 and  Fig. 5).	transcription
53696	1	335148	5	NULL	NULL	0	NULL	VirD2		mutant	mediates			R129G		T-DNA		integration of			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_18_5758_s_221	10482518	These data are reminiscent of the properties of T-DNA integration mediated by a mutant form of VirD2, VirD2R129G (created by replacement of arginine 129 with glycine;  44); in both cases, the efficiency of integration is unaltered compared to the respective wild-type situation while the pattern of integration indicates deletions at the 5' end.	transcription
55149	1	335148	7	NULL	NULL	0	NULL	VirD2		mutant	mediate					T-DNA		integration of			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_18_5758_s_221	10482518	These data are reminiscent of the properties of T-DNA integration mediated by a mutant form of VirD2, VirD2R129G (created by replacement of arginine 129 with glycine;  44); in both cases, the efficiency of integration is unaltered compared to the respective wild-type situation while the pattern of integration indicates deletions at the 5' end.	transcription
55150	2	335148	7	NULL	NULL	0	NULL	VirD2		mutant	mediate			R129G		T-DNA		integration of			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_18_5758_s_221	10482518	These data are reminiscent of the properties of T-DNA integration mediated by a mutant form of VirD2, VirD2R129G (created by replacement of arginine 129 with glycine;  44); in both cases, the efficiency of integration is unaltered compared to the respective wild-type situation while the pattern of integration indicates deletions at the 5' end.	transcription
55151	3	335148	7	NULL	NULL	0	NULL	T-DNA		pattern of;;integration of	indicates									deletion at 5' end	NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_18_5758_s_221	10482518	These data are reminiscent of the properties of T-DNA integration mediated by a mutant form of VirD2, VirD2R129G (created by replacement of arginine 129 with glycine;  44); in both cases, the efficiency of integration is unaltered compared to the respective wild-type situation while the pattern of integration indicates deletions at the 5' end.	transcription
53697	1	335149	5	NULL	NULL	0	NULL	SMN			interacts with					fibrillarin			GAR domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_38645_s_210	11509571	We have found that SMN interacts with the GAR domain of fibrillarin (Figs.  4 and  5), and other studies indicate that SMN also interacts with hnRNP U ( 34), several Sm and Sm-like (Lsm) proteins ( 23,  36,  41,  44,  62), and RNA helicase A ( 30) via glycine/arginine-rich domains.	transcription
53698	2	335149	5	NULL	NULL	0	NULL	SMN			interacts with			glycine/arginine-rich domains		hnRNP U					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38645_s_210	11509571	We have found that SMN interacts with the GAR domain of fibrillarin (Figs.  4 and  5), and other studies indicate that SMN also interacts with hnRNP U ( 34), several Sm and Sm-like (Lsm) proteins ( 23,  36,  41,  44,  62), and RNA helicase A ( 30) via glycine/arginine-rich domains.	transcription
53699	3	335149	5	NULL	NULL	0	NULL	SMN			interacts with			glycine/arginine-rich domains		Sm proteins					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38645_s_210	11509571	We have found that SMN interacts with the GAR domain of fibrillarin (Figs.  4 and  5), and other studies indicate that SMN also interacts with hnRNP U ( 34), several Sm and Sm-like (Lsm) proteins ( 23,  36,  41,  44,  62), and RNA helicase A ( 30) via glycine/arginine-rich domains.	transcription
53700	4	335149	5	NULL	NULL	0	NULL	SMN			interacts with			glycine/arginine-rich domains		Sm-like proteins					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38645_s_210	11509571	We have found that SMN interacts with the GAR domain of fibrillarin (Figs.  4 and  5), and other studies indicate that SMN also interacts with hnRNP U ( 34), several Sm and Sm-like (Lsm) proteins ( 23,  36,  41,  44,  62), and RNA helicase A ( 30) via glycine/arginine-rich domains.	transcription
53701	5	335149	5	NULL	NULL	0	NULL	SMN			interacts with			glycine/arginine-rich domain		RNA helicase A					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_38645_s_210	11509571	We have found that SMN interacts with the GAR domain of fibrillarin (Figs.  4 and  5), and other studies indicate that SMN also interacts with hnRNP U ( 34), several Sm and Sm-like (Lsm) proteins ( 23,  36,  41,  44,  62), and RNA helicase A ( 30) via glycine/arginine-rich domains.	transcription
53702	6	335149	5	NULL	NULL	0	NULL	Lsm			is					Sm-like proteins					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_38645_s_210	11509571	We have found that SMN interacts with the GAR domain of fibrillarin (Figs.  4 and  5), and other studies indicate that SMN also interacts with hnRNP U ( 34), several Sm and Sm-like (Lsm) proteins ( 23,  36,  41,  44,  62), and RNA helicase A ( 30) via glycine/arginine-rich domains.	transcription
55152	1	335149	7	NULL	NULL	0	NULL	SMN			interacts with					fibrillarin			GAR domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_38645_s_210	11509571	We have found that SMN interacts with the GAR domain of fibrillarin (Figs.  4 and  5), and other studies indicate that SMN also interacts with hnRNP U ( 34), several Sm and Sm-like (Lsm) proteins ( 23,  36,  41,  44,  62), and RNA helicase A ( 30) via glycine/arginine-rich domains.	transcription
55153	2	335149	7	NULL	NULL	0	NULL	SMN			interacts with					 hnRNP U			glycine/arginine-rich domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_42_38645_s_210	11509571	We have found that SMN interacts with the GAR domain of fibrillarin (Figs.  4 and  5), and other studies indicate that SMN also interacts with hnRNP U ( 34), several Sm and Sm-like (Lsm) proteins ( 23,  36,  41,  44,  62), and RNA helicase A ( 30) via glycine/arginine-rich domains.	transcription
55169	3	335149	7	NULL	NULL	0	NULL	SMN			interacts with					SM protein			glycine/arginine-rich domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_38645_s_210	11509571	We have found that SMN interacts with the GAR domain of fibrillarin (Figs.  4 and  5), and other studies indicate that SMN also interacts with hnRNP U ( 34), several Sm and Sm-like (Lsm) proteins ( 23,  36,  41,  44,  62), and RNA helicase A ( 30) via glycine/arginine-rich domains.	transcription
55170	4	335149	7	NULL	NULL	0	NULL	SMN			interacts with					Lsm			glycine/arginine-rich domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_38645_s_210	11509571	We have found that SMN interacts with the GAR domain of fibrillarin (Figs.  4 and  5), and other studies indicate that SMN also interacts with hnRNP U ( 34), several Sm and Sm-like (Lsm) proteins ( 23,  36,  41,  44,  62), and RNA helicase A ( 30) via glycine/arginine-rich domains.	transcription
55171	5	335149	7	NULL	NULL	0	NULL	SMN			interacts with					RNA helicase A			glycine/arginine-rich domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_38645_s_210	11509571	We have found that SMN interacts with the GAR domain of fibrillarin (Figs.  4 and  5), and other studies indicate that SMN also interacts with hnRNP U ( 34), several Sm and Sm-like (Lsm) proteins ( 23,  36,  41,  44,  62), and RNA helicase A ( 30) via glycine/arginine-rich domains.	transcription
55172	6	335149	7	NULL	NULL	0	NULL	Lsm			is a type of					Sm-like protein					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_38645_s_210	11509571	We have found that SMN interacts with the GAR domain of fibrillarin (Figs.  4 and  5), and other studies indicate that SMN also interacts with hnRNP U ( 34), several Sm and Sm-like (Lsm) proteins ( 23,  36,  41,  44,  62), and RNA helicase A ( 30) via glycine/arginine-rich domains.	transcription
55173	1	335151	7	NULL	NULL	0	NULL	GCC			encode					glycine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_37_23130_s_46	9287315	The 3 -primer, 5 -gggcggccgcTCAGAAGAGGCC GCCGTCCTTCAGCGTTGTTCTTGATGATGACGT-3 , contains the  NotI site, a stop codon, and 14 amino acids in the C-terminal region of Gi2alpha, except for GCC (underlined), which encodes glycine instead of cysteine at position 352 from the N terminus.	transcription
55174	1	335152	7	NULL	NULL	0	NULL	GCC			encode					glycine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_37_23130_s_49	9287315	The 3 -primer, 5 -gggcggccgcTCAGTAAAGCCC GCCTTCCTTTAAGTTGTT-3 , contains the  NotI site, a stop codon, and nine amino acids in the C-terminal region of Gi3alpha, except for GCC (underlined), which encodes glycine instead of cysteine at position 351 from the N terminus.	transcription
53703	1	335153	5	NULL	NULL	0	NULL	scallop omega-crystallin			forms			Glycine 254;;valine 278;;valine 282		scallop omega-crystallin		altered	NAD pocket		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_52_41064_s_204	10961997	Glycine 254, valine 278, and especially, valine 282 (marked by  arrows and   in Fig.  5) may form an altered NAD pocket in scallop omega-crystallin limiting the binding of NAD required for enzymatic activity (see below and Fig.  8).	transcription
53704	2	335153	5	NULL	NULL	0	NULL	NAD		binding of	is required for					scallop omega-crystallin		enzymatic activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_52_41064_s_204	10961997	Glycine 254, valine 278, and especially, valine 282 (marked by  arrows and   in Fig.  5) may form an altered NAD pocket in scallop omega-crystallin limiting the binding of NAD required for enzymatic activity (see below and Fig.  8).	transcription
53705	3	335153	5	NULL	NULL	0	NULL	statement 1			limits					NAD		binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_52_41064_s_204	10961997	Glycine 254, valine 278, and especially, valine 282 (marked by  arrows and   in Fig.  5) may form an altered NAD pocket in scallop omega-crystallin limiting the binding of NAD required for enzymatic activity (see below and Fig.  8).	transcription
55175	1	335153	7	NULL	NULL	0	NULL				form		may	Glycine 254, valine 278, valine 282		omega-crystallin		scallop	altered NAD pocket  		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_52_41064_s_204	10961997	Glycine 254, valine 278, and especially, valine 282 (marked by  arrows and   in Fig.  5) may form an altered NAD pocket in scallop omega-crystallin limiting the binding of NAD required for enzymatic activity (see below and Fig.  8).	transcription
55176	2	335153	7	NULL	NULL	0	NULL	statement 1			limit					NAD		binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_52_41064_s_204	10961997	Glycine 254, valine 278, and especially, valine 282 (marked by  arrows and   in Fig.  5) may form an altered NAD pocket in scallop omega-crystallin limiting the binding of NAD required for enzymatic activity (see below and Fig.  8).	transcription
55177	3	335153	7	NULL	NULL	0	NULL	statement 2			is required for					enzymatic activity					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_52_41064_s_204	10961997	Glycine 254, valine 278, and especially, valine 282 (marked by  arrows and   in Fig.  5) may form an altered NAD pocket in scallop omega-crystallin limiting the binding of NAD required for enzymatic activity (see below and Fig.  8).	transcription
53706	1	335155	5	NULL	NULL	0	NULL	glycine			stimulates					pre-MG		activation of	D151G		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_16_9695_s_248	9545304	4) Instead of inhibition of the activation, glycine actually stimulated the activation of pre-MG(D151G) (Fig.  5), which is very similar to the observation that methylamine inhibits trypsin hydrolysis of specific substrates and stimulates the enzyme activity toward nonspecific substrates ( 26).	transcription
53707	2	335155	5	NULL	NULL	0	NULL	methylamine			inhibits					substrates		hydrolysis of;;specific			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_16_9695_s_248	9545304	4) Instead of inhibition of the activation, glycine actually stimulated the activation of pre-MG(D151G) (Fig.  5), which is very similar to the observation that methylamine inhibits trypsin hydrolysis of specific substrates and stimulates the enzyme activity toward nonspecific substrates ( 26).	transcription
53708	3	335155	5	NULL	NULL	0	NULL	statement 2			stimulates					substrates		enzyme activity toward;;nonspecific			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_16_9695_s_248	9545304	4) Instead of inhibition of the activation, glycine actually stimulated the activation of pre-MG(D151G) (Fig.  5), which is very similar to the observation that methylamine inhibits trypsin hydrolysis of specific substrates and stimulates the enzyme activity toward nonspecific substrates ( 26).	transcription
55178	1	335155	7	NULL	NULL	0	NULL	glycine			stimulate					 pre-MG(D151G)		activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_16_9695_s_248	9545304	4) Instead of inhibition of the activation, glycine actually stimulated the activation of pre-MG(D151G) (Fig.  5), which is very similar to the observation that methylamine inhibits trypsin hydrolysis of specific substrates and stimulates the enzyme activity toward nonspecific substrates ( 26).	transcription
55179	3	335155	7	NULL	NULL	0	NULL	methylamine 			inhibits					statement 2					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_16_9695_s_248	9545304	4) Instead of inhibition of the activation, glycine actually stimulated the activation of pre-MG(D151G) (Fig.  5), which is very similar to the observation that methylamine inhibits trypsin hydrolysis of specific substrates and stimulates the enzyme activity toward nonspecific substrates ( 26).	transcription
55180	2	335155	7	NULL	NULL	0	NULL	trypsin			hydrolyse					substrates					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_16_9695_s_248	9545304	4) Instead of inhibition of the activation, glycine actually stimulated the activation of pre-MG(D151G) (Fig.  5), which is very similar to the observation that methylamine inhibits trypsin hydrolysis of specific substrates and stimulates the enzyme activity toward nonspecific substrates ( 26).	transcription
55181	4	335155	7	NULL	NULL	0	NULL	statement 2			stimulate					enzyme activity					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_16_9695_s_248	9545304	4) Instead of inhibition of the activation, glycine actually stimulated the activation of pre-MG(D151G) (Fig.  5), which is very similar to the observation that methylamine inhibits trypsin hydrolysis of specific substrates and stimulates the enzyme activity toward nonspecific substrates ( 26).	transcription
53709	1	335156	5	NULL	NULL	0	NULL	Li+			is substituted for					Na+					NULL	external medium	0	NULL	NULL	NULL	gw60_jneurosci_17_12_4580_s_145	9169519	This does not occur (1) in oocytes in which GLYT1b was not expressed; (2) when the GLYT1b is inhibited by substituting Li+ for Na+ in the external medium; (3) when glycine is replaced by D-serine in the external medium; (4) when GLYT1b is saturated by sarcosine; or (5) when membrane voltage changes alter the carrier function.	transcription
53710	2	335156	5	NULL	NULL	0	NULL	statement 1			inhibits					GLYT1b					NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_12_4580_s_145	9169519	This does not occur (1) in oocytes in which GLYT1b was not expressed; (2) when the GLYT1b is inhibited by substituting Li+ for Na+ in the external medium; (3) when glycine is replaced by D-serine in the external medium; (4) when GLYT1b is saturated by sarcosine; or (5) when membrane voltage changes alter the carrier function.	transcription
53711	3	335156	5	NULL	NULL	0	NULL	GLYT1b			is saturated by					sarcosine					NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_17_12_4580_s_145	9169519	This does not occur (1) in oocytes in which GLYT1b was not expressed; (2) when the GLYT1b is inhibited by substituting Li+ for Na+ in the external medium; (3) when glycine is replaced by D-serine in the external medium; (4) when GLYT1b is saturated by sarcosine; or (5) when membrane voltage changes alter the carrier function.	transcription
53712	4	335156	5	NULL	NULL	0	NULL	membrane voltage		changes in	alter					carrier		function of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_12_4580_s_145	9169519	This does not occur (1) in oocytes in which GLYT1b was not expressed; (2) when the GLYT1b is inhibited by substituting Li+ for Na+ in the external medium; (3) when glycine is replaced by D-serine in the external medium; (4) when GLYT1b is saturated by sarcosine; or (5) when membrane voltage changes alter the carrier function.	transcription
53800	1	335158	5	NULL	NULL	0	NULL	NMDA			activates					NMDARs					NULL	cerebrocortical neurons	0	NULL	NULL	NULL	gw60_jneurosci_21_20_7985_s_63	11588171	Activation of NMDARs in cerebrocortical neurons and transfected HEK 293 cells expressing heteromeric NMDARs was induced by adding 200 muM NMDA, 10 muM glycine, and 2.5 mM calcium in nominally Mg2+-free Hank's solution at 37 degrees C for 5 min.	transcription
53801	2	335158	5	NULL	NULL	0	NULL	NMDA			activates					NMDARs					NULL	transfected HEK 293 cells expressing heteromeric NMDARs 	0	NULL	NULL	NULL	gw60_jneurosci_21_20_7985_s_63	11588171	Activation of NMDARs in cerebrocortical neurons and transfected HEK 293 cells expressing heteromeric NMDARs was induced by adding 200 muM NMDA, 10 muM glycine, and 2.5 mM calcium in nominally Mg2+-free Hank's solution at 37 degrees C for 5 min.	transcription
53802	3	335158	5	NULL	NULL	0	NULL	glycine			activates					NMDARs					NULL	cerebrocortical neurons	0	NULL	NULL	NULL	gw60_jneurosci_21_20_7985_s_63	11588171	Activation of NMDARs in cerebrocortical neurons and transfected HEK 293 cells expressing heteromeric NMDARs was induced by adding 200 muM NMDA, 10 muM glycine, and 2.5 mM calcium in nominally Mg2+-free Hank's solution at 37 degrees C for 5 min.	transcription
53803	4	335158	5	NULL	NULL	0	NULL	glycine			activates					NMDARs					NULL	transfected HEK 293 cells expressing heteromeric NMDARs	0	NULL	NULL	NULL	gw60_jneurosci_21_20_7985_s_63	11588171	Activation of NMDARs in cerebrocortical neurons and transfected HEK 293 cells expressing heteromeric NMDARs was induced by adding 200 muM NMDA, 10 muM glycine, and 2.5 mM calcium in nominally Mg2+-free Hank's solution at 37 degrees C for 5 min.	transcription
53804	5	335158	5	NULL	NULL	0	NULL	calcium			activates					NMDARs					NULL	cerebrocortical neurons	0	NULL	NULL	NULL	gw60_jneurosci_21_20_7985_s_63	11588171	Activation of NMDARs in cerebrocortical neurons and transfected HEK 293 cells expressing heteromeric NMDARs was induced by adding 200 muM NMDA, 10 muM glycine, and 2.5 mM calcium in nominally Mg2+-free Hank's solution at 37 degrees C for 5 min.	transcription
53805	6	335158	5	NULL	NULL	0	NULL	calcium			activates					NMDARs					NULL	transfected HEK 293 cells expressing heteromeric NMDARs	0	NULL	NULL	NULL	gw60_jneurosci_21_20_7985_s_63	11588171	Activation of NMDARs in cerebrocortical neurons and transfected HEK 293 cells expressing heteromeric NMDARs was induced by adding 200 muM NMDA, 10 muM glycine, and 2.5 mM calcium in nominally Mg2+-free Hank's solution at 37 degrees C for 5 min.	transcription
56145	1	335158	7	NULL	NULL	0	NULL	HEK 293 cells 			express					heteromeric NMDARs					NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_20_7985_s_63	11588171	Activation of NMDARs in cerebrocortical neurons and transfected HEK 293 cells expressing heteromeric NMDARs was induced by adding 200 muM NMDA, 10 muM glycine, and 2.5 mM calcium in nominally Mg2+-free Hank's solution at 37 degrees C for 5 min.	transcription
53806	1	335159	5	NULL	NULL	0	NULL	group II metabotropic glutamate receptors			is coupled with					Gi					NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_4_1257_s_220	11160396	The enhancement because of forskolin treatment was inhibited by a 5 min pretreatment with (2S, 1'R, 2'R, 3'R)-2-2(2,3-dicarboxyclopropyl)glycine, an agonist of group II metabotropic glutamate receptors that is coupled with Gi and negatively regulates adenylate cyclase (data not shown).	transcription
53807	2	335159	5	NULL	NULL	0	NULL	(2S, 1'R, 2'R, 3'R)-2-2(2,3-dicarboxyclopropyl)glycine			is an agonist of					statement 1					NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_4_1257_s_220	11160396	The enhancement because of forskolin treatment was inhibited by a 5 min pretreatment with (2S, 1'R, 2'R, 3'R)-2-2(2,3-dicarboxyclopropyl)glycine, an agonist of group II metabotropic glutamate receptors that is coupled with Gi and negatively regulates adenylate cyclase (data not shown).	transcription
53808	3	335159	5	NULL	NULL	0	NULL	statement 1			regulates		negatively			adenylate cyclase					NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_4_1257_s_220	11160396	The enhancement because of forskolin treatment was inhibited by a 5 min pretreatment with (2S, 1'R, 2'R, 3'R)-2-2(2,3-dicarboxyclopropyl)glycine, an agonist of group II metabotropic glutamate receptors that is coupled with Gi and negatively regulates adenylate cyclase (data not shown).	transcription
55182	1	335159	7	NULL	NULL	0	NULL	glutamate receptors			coupled with					Gi					NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_4_1257_s_220	11160396	The enhancement because of forskolin treatment was inhibited by a 5 min pretreatment with (2S, 1'R, 2'R, 3'R)-2-2(2,3-dicarboxyclopropyl)glycine, an agonist of group II metabotropic glutamate receptors that is coupled with Gi and negatively regulates adenylate cyclase (data not shown).	transcription
55183	2	335159	7	NULL	NULL	0	NULL	glutamate receptors			is a type of					group II metabotropic receptor					NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_4_1257_s_220	11160396	The enhancement because of forskolin treatment was inhibited by a 5 min pretreatment with (2S, 1'R, 2'R, 3'R)-2-2(2,3-dicarboxyclopropyl)glycine, an agonist of group II metabotropic glutamate receptors that is coupled with Gi and negatively regulates adenylate cyclase (data not shown).	transcription
55184	3	335159	7	NULL	NULL	0	NULL	(2S, 1'R, 2'R, 3'R)-2-2(2,3-dicarboxyclopropyl)glycine			is an agonist of					statement 1					NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_4_1257_s_220	11160396	The enhancement because of forskolin treatment was inhibited by a 5 min pretreatment with (2S, 1'R, 2'R, 3'R)-2-2(2,3-dicarboxyclopropyl)glycine, an agonist of group II metabotropic glutamate receptors that is coupled with Gi and negatively regulates adenylate cyclase (data not shown).	transcription
55185	4	335159	7	NULL	NULL	0	NULL	statement 1			regulates		negatively			adenylate cyclase					NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_4_1257_s_220	11160396	The enhancement because of forskolin treatment was inhibited by a 5 min pretreatment with (2S, 1'R, 2'R, 3'R)-2-2(2,3-dicarboxyclopropyl)glycine, an agonist of group II metabotropic glutamate receptors that is coupled with Gi and negatively regulates adenylate cyclase (data not shown).	transcription
55186	1	335160	7	NULL	NULL	0	NULL	GABA			induce					[Ca2+]i 		increase of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_21_7905_s_191	11050110	However, on average, 24.5  plus-or-minus  6% ( n = 5) of the GABA-induced [Ca2+]i increase and 21.0  plus-or-minus  3.8% ( n = 4) of the glycine-induced [Ca2+]i transient persisted even during exposure to the drug for time periods of >1 hr (Fig.  8 A, B).	transcription
55187	2	335160	7	NULL	NULL	0	NULL	 glycine			induce					[Ca2+]i					NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_21_7905_s_191	11050110	However, on average, 24.5  plus-or-minus  6% ( n = 5) of the GABA-induced [Ca2+]i increase and 21.0  plus-or-minus  3.8% ( n = 4) of the glycine-induced [Ca2+]i transient persisted even during exposure to the drug for time periods of >1 hr (Fig.  8 A, B).	transcription
53856	1	335161	5	NULL	NULL	0	NULL	spermine		stimulation of	is independent of					glycine					NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1026_s_22	10454474	The glycine-independent form of spermine stimulation may involve relief of proton inhibition, and both processes are influenced by the alternatively spliced insert encoded by exon 5 in the NR1 subunit (Zheng et al., 1994  ; Traynelis et al., 1995  ).	transcription
53866	2	335161	5	NULL	NULL	0	NULL	statement 1			involves		may			proton		relief of;;inhibition of			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1026_s_22	10454474	The glycine-independent form of spermine stimulation may involve relief of proton inhibition, and both processes are influenced by the alternatively spliced insert encoded by exon 5 in the NR1 subunit (Zheng et al., 1994  ; Traynelis et al., 1995  ).	transcription
53867	3	335161	5	NULL	NULL	0	NULL	alternatively spliced insert			is encoded by					NR1 subunit				exon 5	NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1026_s_22	10454474	The glycine-independent form of spermine stimulation may involve relief of proton inhibition, and both processes are influenced by the alternatively spliced insert encoded by exon 5 in the NR1 subunit (Zheng et al., 1994  ; Traynelis et al., 1995  ).	transcription
53868	4	335161	5	NULL	NULL	0	NULL	statement 3			influences					statement 1					NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1026_s_22	10454474	The glycine-independent form of spermine stimulation may involve relief of proton inhibition, and both processes are influenced by the alternatively spliced insert encoded by exon 5 in the NR1 subunit (Zheng et al., 1994  ; Traynelis et al., 1995  ).	transcription
53869	5	335161	5	NULL	NULL	0	NULL	statement 3			influences					statement 2					NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1026_s_22	10454474	The glycine-independent form of spermine stimulation may involve relief of proton inhibition, and both processes are influenced by the alternatively spliced insert encoded by exon 5 in the NR1 subunit (Zheng et al., 1994  ; Traynelis et al., 1995  ).	transcription
55188	1	335161	7	NULL	NULL	0	NULL	spermine		stimulation of	is independent of					glycine					NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1026_s_22	10454474	The glycine-independent form of spermine stimulation may involve relief of proton inhibition, and both processes are influenced by the alternatively spliced insert encoded by exon 5 in the NR1 subunit (Zheng et al., 1994  ; Traynelis et al., 1995  ).	transcription
55189	2	335161	7	NULL	NULL	0	NULL	statement 1			involve		may			proton 		relief of;; inhibition of			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1026_s_22	10454474	The glycine-independent form of spermine stimulation may involve relief of proton inhibition, and both processes are influenced by the alternatively spliced insert encoded by exon 5 in the NR1 subunit (Zheng et al., 1994  ; Traynelis et al., 1995  ).	transcription
55190	3	335161	7	NULL	NULL	0	NULL				encode				exon 5				NR1 subunit	alternatively spliced insert	NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1026_s_22	10454474	The glycine-independent form of spermine stimulation may involve relief of proton inhibition, and both processes are influenced by the alternatively spliced insert encoded by exon 5 in the NR1 subunit (Zheng et al., 1994  ; Traynelis et al., 1995  ).	transcription
55191	4	335161	7	NULL	NULL	0	NULL	statement 3			influence					statement 1					NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1026_s_22	10454474	The glycine-independent form of spermine stimulation may involve relief of proton inhibition, and both processes are influenced by the alternatively spliced insert encoded by exon 5 in the NR1 subunit (Zheng et al., 1994  ; Traynelis et al., 1995  ).	transcription
55192	5	335161	7	NULL	NULL	0	NULL	statement 3			influence					statement 2					NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1026_s_22	10454474	The glycine-independent form of spermine stimulation may involve relief of proton inhibition, and both processes are influenced by the alternatively spliced insert encoded by exon 5 in the NR1 subunit (Zheng et al., 1994  ; Traynelis et al., 1995  ).	transcription
53870	1	335162	5	NULL	NULL	0	NULL	NMDA receptors		functional	gates					inward currents					NULL	Xenopus oocytes	NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_292_1_215_s_289	10604951	As previously reported (Hess et al., 1996  ), expression of human NR1a/NR2A or NR1a/NR2B subunits in  Xenopus oocytes resulted in functional NMDA receptors that gated inward currents of 50 to 500 nA on coperfusion of 100 muM NMDA and 1 muM glycine (Fig.  5) when oocytes were voltage-clamped at negative potentials.	transcription
53871	2	335162	5	NULL	NULL	0	NULL	NR1a/NR2A subunits		expression of	results in					NMDA receptors		functional			NULL	Xenopus oocytes	0	NULL	NULL	NULL	gw60_jpharmacolexpther_292_1_215_s_289	10604951	As previously reported (Hess et al., 1996  ), expression of human NR1a/NR2A or NR1a/NR2B subunits in  Xenopus oocytes resulted in functional NMDA receptors that gated inward currents of 50 to 500 nA on coperfusion of 100 muM NMDA and 1 muM glycine (Fig.  5) when oocytes were voltage-clamped at negative potentials.	transcription
53872	3	335162	5	NULL	NULL	0	NULL	NR1a/NR2B subunits		expression of	results in					NMDA receptors		functional			NULL	Xenopus oocytes	0	NULL	NULL	NULL	gw60_jpharmacolexpther_292_1_215_s_289	10604951	As previously reported (Hess et al., 1996  ), expression of human NR1a/NR2A or NR1a/NR2B subunits in  Xenopus oocytes resulted in functional NMDA receptors that gated inward currents of 50 to 500 nA on coperfusion of 100 muM NMDA and 1 muM glycine (Fig.  5) when oocytes were voltage-clamped at negative potentials.	transcription
55193	1	335162	7	NULL	NULL	0	NULL			human	expressed in			NR1a/NR2A subunit		oocytes		Xenopus			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_292_1_215_s_289	10604951	As previously reported (Hess et al., 1996  ), expression of human NR1a/NR2A or NR1a/NR2B subunits in  Xenopus oocytes resulted in functional NMDA receptors that gated inward currents of 50 to 500 nA on coperfusion of 100 muM NMDA and 1 muM glycine (Fig.  5) when oocytes were voltage-clamped at negative potentials.	transcription
55194	2	335162	7	NULL	NULL	0	NULL			human	expressed in			NR1a/NR2B subunit		oocytes		Xenopus			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_292_1_215_s_289	10604951	As previously reported (Hess et al., 1996  ), expression of human NR1a/NR2A or NR1a/NR2B subunits in  Xenopus oocytes resulted in functional NMDA receptors that gated inward currents of 50 to 500 nA on coperfusion of 100 muM NMDA and 1 muM glycine (Fig.  5) when oocytes were voltage-clamped at negative potentials.	transcription
55195	3	335162	7	NULL	NULL	0	NULL	statement 1			result in					NMDA receptors		functional			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_292_1_215_s_289	10604951	As previously reported (Hess et al., 1996  ), expression of human NR1a/NR2A or NR1a/NR2B subunits in  Xenopus oocytes resulted in functional NMDA receptors that gated inward currents of 50 to 500 nA on coperfusion of 100 muM NMDA and 1 muM glycine (Fig.  5) when oocytes were voltage-clamped at negative potentials.	transcription
55196	4	335162	7	NULL	NULL	0	NULL	statement 2			result in					NMDA receptor		functional			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_292_1_215_s_289	10604951	As previously reported (Hess et al., 1996  ), expression of human NR1a/NR2A or NR1a/NR2B subunits in  Xenopus oocytes resulted in functional NMDA receptors that gated inward currents of 50 to 500 nA on coperfusion of 100 muM NMDA and 1 muM glycine (Fig.  5) when oocytes were voltage-clamped at negative potentials.	transcription
53873	1	335163	5	NULL	NULL	0	NULL	BP		transport of	is induced by					epinephrine					NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_293_1_128_s_141	10734162	After perfusion of the lumen with Ringer's solution containing BP in the presence of these compounds, epinephrine was added to the perfusate at a concentration of 0.1 mM and perfusion was continued for an additional 30 min. Glycyl-L-alanine, glycyl-L-leucine, glycylsarcosine, and glycyl-glycyl-glycine reduced the extent of epinephrine-induced BP transport by 80 to 90% (Table  5).	transcription
53874	2	335163	5	NULL	NULL	0	NULL	Glycyl-L-alanine			reduces					statement 1					NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_293_1_128_s_141	10734162	After perfusion of the lumen with Ringer's solution containing BP in the presence of these compounds, epinephrine was added to the perfusate at a concentration of 0.1 mM and perfusion was continued for an additional 30 min. Glycyl-L-alanine, glycyl-L-leucine, glycylsarcosine, and glycyl-glycyl-glycine reduced the extent of epinephrine-induced BP transport by 80 to 90% (Table  5).	transcription
53875	3	335163	5	NULL	NULL	0	NULL	glycyl-L-leucine			reduces					statement 1					NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_293_1_128_s_141	10734162	After perfusion of the lumen with Ringer's solution containing BP in the presence of these compounds, epinephrine was added to the perfusate at a concentration of 0.1 mM and perfusion was continued for an additional 30 min. Glycyl-L-alanine, glycyl-L-leucine, glycylsarcosine, and glycyl-glycyl-glycine reduced the extent of epinephrine-induced BP transport by 80 to 90% (Table  5).	transcription
53876	4	335163	5	NULL	NULL	0	NULL	glycylsarcosine			reduces					statement 1					NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_293_1_128_s_141	10734162	After perfusion of the lumen with Ringer's solution containing BP in the presence of these compounds, epinephrine was added to the perfusate at a concentration of 0.1 mM and perfusion was continued for an additional 30 min. Glycyl-L-alanine, glycyl-L-leucine, glycylsarcosine, and glycyl-glycyl-glycine reduced the extent of epinephrine-induced BP transport by 80 to 90% (Table  5).	transcription
53877	5	335163	5	NULL	NULL	0	NULL	glycyl-glycyl-glycine			reduces					statement 1					NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_293_1_128_s_141	10734162	After perfusion of the lumen with Ringer's solution containing BP in the presence of these compounds, epinephrine was added to the perfusate at a concentration of 0.1 mM and perfusion was continued for an additional 30 min. Glycyl-L-alanine, glycyl-L-leucine, glycylsarcosine, and glycyl-glycyl-glycine reduced the extent of epinephrine-induced BP transport by 80 to 90% (Table  5).	transcription
55197	1	335163	7	NULL	NULL	0	NULL	epinephrine			induce					BP		transport of			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_293_1_128_s_141	10734162	After perfusion of the lumen with Ringer's solution containing BP in the presence of these compounds, epinephrine was added to the perfusate at a concentration of 0.1 mM and perfusion was continued for an additional 30 min. Glycyl-L-alanine, glycyl-L-leucine, glycylsarcosine, and glycyl-glycyl-glycine reduced the extent of epinephrine-induced BP transport by 80 to 90% (Table  5).	transcription
55198	2	335163	7	NULL	NULL	0	NULL	Glycyl-L-alanine			reduce					statement 1					NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_293_1_128_s_141	10734162	After perfusion of the lumen with Ringer's solution containing BP in the presence of these compounds, epinephrine was added to the perfusate at a concentration of 0.1 mM and perfusion was continued for an additional 30 min. Glycyl-L-alanine, glycyl-L-leucine, glycylsarcosine, and glycyl-glycyl-glycine reduced the extent of epinephrine-induced BP transport by 80 to 90% (Table  5).	transcription
55199	3	335163	7	NULL	NULL	0	NULL	glycyl-L-leucine			reduce					statement 1					NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_293_1_128_s_141	10734162	After perfusion of the lumen with Ringer's solution containing BP in the presence of these compounds, epinephrine was added to the perfusate at a concentration of 0.1 mM and perfusion was continued for an additional 30 min. Glycyl-L-alanine, glycyl-L-leucine, glycylsarcosine, and glycyl-glycyl-glycine reduced the extent of epinephrine-induced BP transport by 80 to 90% (Table  5).	transcription
55200	4	335163	7	NULL	NULL	0	NULL	glycylsarcosine			reduce					statement 1					NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_293_1_128_s_141	10734162	After perfusion of the lumen with Ringer's solution containing BP in the presence of these compounds, epinephrine was added to the perfusate at a concentration of 0.1 mM and perfusion was continued for an additional 30 min. Glycyl-L-alanine, glycyl-L-leucine, glycylsarcosine, and glycyl-glycyl-glycine reduced the extent of epinephrine-induced BP transport by 80 to 90% (Table  5).	transcription
55201	5	335163	7	NULL	NULL	0	NULL	glycyl-glycyl-glycine			reduce					statement 1					NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_293_1_128_s_141	10734162	After perfusion of the lumen with Ringer's solution containing BP in the presence of these compounds, epinephrine was added to the perfusate at a concentration of 0.1 mM and perfusion was continued for an additional 30 min. Glycyl-L-alanine, glycyl-L-leucine, glycylsarcosine, and glycyl-glycyl-glycine reduced the extent of epinephrine-induced BP transport by 80 to 90% (Table  5).	transcription
55202	1	335164	7	NULL	NULL	0	NULL			Arabidopsis thaliana	encode				Atgrp7 	glycine-rich RNA-binding proteins					NULL		0	NULL	NULL	NULL	gw60_pnas_94_16_8515_s_27	9238008	Gene- and strand-specific antisense probes that distinguish between the  Arabidopsis thaliana genes  Atgrp7 ( 23), also designated  ccr2 ( 24), and  Atgrp8 ( 23), also designated ccr1 ( 24), both encoding glycine-rich RNA-binding proteins with 75% sequence identity ( 23,  24), were derived from the 5  untranslated regions.	transcription
55203	2	335164	7	NULL	NULL	0	NULL			Arabidopsis thaliana	encode				Atgrp8	glycine-rich RNA-binding proteins					NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_16_8515_s_27	9238008	Gene- and strand-specific antisense probes that distinguish between the  Arabidopsis thaliana genes  Atgrp7 ( 23), also designated  ccr2 ( 24), and  Atgrp8 ( 23), also designated ccr1 ( 24), both encoding glycine-rich RNA-binding proteins with 75% sequence identity ( 23,  24), were derived from the 5  untranslated regions.	transcription
55204	3	335164	7	NULL	NULL	0	NULL				is designated as				Atgrp7	ccr2					NULL		0	NULL	NULL	NULL	gw60_pnas_94_16_8515_s_27	9238008	Gene- and strand-specific antisense probes that distinguish between the  Arabidopsis thaliana genes  Atgrp7 ( 23), also designated  ccr2 ( 24), and  Atgrp8 ( 23), also designated ccr1 ( 24), both encoding glycine-rich RNA-binding proteins with 75% sequence identity ( 23,  24), were derived from the 5  untranslated regions.	transcription
55205	4	335164	7	NULL	NULL	0	NULL				is designated as				Atgrp8	ccr1					NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_16_8515_s_27	9238008	Gene- and strand-specific antisense probes that distinguish between the  Arabidopsis thaliana genes  Atgrp7 ( 23), also designated  ccr2 ( 24), and  Atgrp8 ( 23), also designated ccr1 ( 24), both encoding glycine-rich RNA-binding proteins with 75% sequence identity ( 23,  24), were derived from the 5  untranslated regions.	transcription
53878	1	335165	5	NULL	NULL	0	NULL	glycine betaine			is a type of					stabilizing cosolutes					NULL		0	NULL	NULL	NULL	abs-batch0530-0539_photosynth-res_65_1_16228469_s_6	16228469	Presence of stabilizing cosolutes (glycine  betaine, sucrose) or addition of donor-side cofactors (bicarbonate, chloride,  calcium) to PS II membranes before heating (47 degrees C, 5 min) diminishes  J-P phase suppression and prevents dip appearance, whereas the addition  after heating is without effect.	transcription
53879	2	335165	5	NULL	NULL	0	NULL	sucrose			is a type of					stabilizing cosolutes					NULL		0	NULL	NULL	NULL	abs-batch0530-0539_photosynth-res_65_1_16228469_s_6	16228469	Presence of stabilizing cosolutes (glycine  betaine, sucrose) or addition of donor-side cofactors (bicarbonate, chloride,  calcium) to PS II membranes before heating (47 degrees C, 5 min) diminishes  J-P phase suppression and prevents dip appearance, whereas the addition  after heating is without effect.	transcription
53880	3	335165	5	NULL	NULL	0	NULL	bicarbonate			is a type of					donor-side cofactors					NULL		0	NULL	NULL	NULL	abs-batch0530-0539_photosynth-res_65_1_16228469_s_6	16228469	Presence of stabilizing cosolutes (glycine  betaine, sucrose) or addition of donor-side cofactors (bicarbonate, chloride,  calcium) to PS II membranes before heating (47 degrees C, 5 min) diminishes  J-P phase suppression and prevents dip appearance, whereas the addition  after heating is without effect.	transcription
53881	4	335165	5	NULL	NULL	0	NULL	chloride			is a type of					donor-side cofactors					NULL		0	NULL	NULL	NULL	abs-batch0530-0539_photosynth-res_65_1_16228469_s_6	16228469	Presence of stabilizing cosolutes (glycine  betaine, sucrose) or addition of donor-side cofactors (bicarbonate, chloride,  calcium) to PS II membranes before heating (47 degrees C, 5 min) diminishes  J-P phase suppression and prevents dip appearance, whereas the addition  after heating is without effect.	transcription
53882	5	335165	5	NULL	NULL	0	NULL	calcium			is a type of					donor-side cofactors					NULL		0	NULL	NULL	NULL	abs-batch0530-0539_photosynth-res_65_1_16228469_s_6	16228469	Presence of stabilizing cosolutes (glycine  betaine, sucrose) or addition of donor-side cofactors (bicarbonate, chloride,  calcium) to PS II membranes before heating (47 degrees C, 5 min) diminishes  J-P phase suppression and prevents dip appearance, whereas the addition  after heating is without effect.	transcription
53884	6	335165	5	NULL	NULL	0	NULL	glycine betaine		presence of	diminishes					J-P phase		suppression of			NULL	PS II membranes	NULL	NULL	NULL	NULL	abs-batch0530-0539_photosynth-res_65_1_16228469_s_6	16228469	Presence of stabilizing cosolutes (glycine  betaine, sucrose) or addition of donor-side cofactors (bicarbonate, chloride,  calcium) to PS II membranes before heating (47 degrees C, 5 min) diminishes  J-P phase suppression and prevents dip appearance, whereas the addition  after heating is without effect.	transcription
53885	7	335165	5	NULL	NULL	0	NULL	statement 6			occurs before					heating					NULL	PS II membranes	NULL	NULL	NULL	NULL	abs-batch0530-0539_photosynth-res_65_1_16228469_s_6	16228469	Presence of stabilizing cosolutes (glycine  betaine, sucrose) or addition of donor-side cofactors (bicarbonate, chloride,  calcium) to PS II membranes before heating (47 degrees C, 5 min) diminishes  J-P phase suppression and prevents dip appearance, whereas the addition  after heating is without effect.	transcription
53886	8	335165	5	NULL	NULL	0	NULL	statement 6			prevents					dip appearance					NULL	PS II membranes	NULL	NULL	NULL	NULL	abs-batch0530-0539_photosynth-res_65_1_16228469_s_6	16228469	Presence of stabilizing cosolutes (glycine  betaine, sucrose) or addition of donor-side cofactors (bicarbonate, chloride,  calcium) to PS II membranes before heating (47 degrees C, 5 min) diminishes  J-P phase suppression and prevents dip appearance, whereas the addition  after heating is without effect.	transcription
53887	9	335165	5	NULL	NULL	0	NULL	sucrose		presence of	diminishes					J-P phase		suppression of			NULL	PS II membranes	0	NULL	NULL	NULL	abs-batch0530-0539_photosynth-res_65_1_16228469_s_6	16228469	Presence of stabilizing cosolutes (glycine  betaine, sucrose) or addition of donor-side cofactors (bicarbonate, chloride,  calcium) to PS II membranes before heating (47 degrees C, 5 min) diminishes  J-P phase suppression and prevents dip appearance, whereas the addition  after heating is without effect.	transcription
53888	10	335165	5	NULL	NULL	0	NULL	statement 9			occurs before					heating					NULL	PS II membranes	0	NULL	NULL	NULL	abs-batch0530-0539_photosynth-res_65_1_16228469_s_6	16228469	Presence of stabilizing cosolutes (glycine  betaine, sucrose) or addition of donor-side cofactors (bicarbonate, chloride,  calcium) to PS II membranes before heating (47 degrees C, 5 min) diminishes  J-P phase suppression and prevents dip appearance, whereas the addition  after heating is without effect.	transcription
53889	11	335165	5	NULL	NULL	0	NULL	statement 9			prevents					dip appearance					NULL	PS II membranes	NULL	NULL	NULL	NULL	abs-batch0530-0539_photosynth-res_65_1_16228469_s_6	16228469	Presence of stabilizing cosolutes (glycine  betaine, sucrose) or addition of donor-side cofactors (bicarbonate, chloride,  calcium) to PS II membranes before heating (47 degrees C, 5 min) diminishes  J-P phase suppression and prevents dip appearance, whereas the addition  after heating is without effect.	transcription
53890	12	335165	5	NULL	NULL	0	NULL	bicarbonate		addition of	diminishes					J-P phase		suppression of			NULL	PS II membranes	NULL	NULL	NULL	NULL	abs-batch0530-0539_photosynth-res_65_1_16228469_s_6	16228469	Presence of stabilizing cosolutes (glycine  betaine, sucrose) or addition of donor-side cofactors (bicarbonate, chloride,  calcium) to PS II membranes before heating (47 degrees C, 5 min) diminishes  J-P phase suppression and prevents dip appearance, whereas the addition  after heating is without effect.	transcription
53891	13	335165	5	NULL	NULL	0	NULL	statement 12			occurs before					heating					NULL	PS II membranes	NULL	NULL	NULL	NULL	abs-batch0530-0539_photosynth-res_65_1_16228469_s_6	16228469	Presence of stabilizing cosolutes (glycine  betaine, sucrose) or addition of donor-side cofactors (bicarbonate, chloride,  calcium) to PS II membranes before heating (47 degrees C, 5 min) diminishes  J-P phase suppression and prevents dip appearance, whereas the addition  after heating is without effect.	transcription
53892	14	335165	5	NULL	NULL	0	NULL	statement 12			prevents					dip appearance					NULL	PS II membranes	0	NULL	NULL	NULL	abs-batch0530-0539_photosynth-res_65_1_16228469_s_6	16228469	Presence of stabilizing cosolutes (glycine  betaine, sucrose) or addition of donor-side cofactors (bicarbonate, chloride,  calcium) to PS II membranes before heating (47 degrees C, 5 min) diminishes  J-P phase suppression and prevents dip appearance, whereas the addition  after heating is without effect.	transcription
53893	15	335165	5	NULL	NULL	0	NULL	chloride		addition of	diminishes					J-P phase		suppression of			NULL	PS II membranes	0	NULL	NULL	NULL	abs-batch0530-0539_photosynth-res_65_1_16228469_s_6	16228469	Presence of stabilizing cosolutes (glycine  betaine, sucrose) or addition of donor-side cofactors (bicarbonate, chloride,  calcium) to PS II membranes before heating (47 degrees C, 5 min) diminishes  J-P phase suppression and prevents dip appearance, whereas the addition  after heating is without effect.	transcription
53894	16	335165	5	NULL	NULL	0	NULL	statement 15			occurs before					heating					NULL	PS II membranes	0	NULL	NULL	NULL	abs-batch0530-0539_photosynth-res_65_1_16228469_s_6	16228469	Presence of stabilizing cosolutes (glycine  betaine, sucrose) or addition of donor-side cofactors (bicarbonate, chloride,  calcium) to PS II membranes before heating (47 degrees C, 5 min) diminishes  J-P phase suppression and prevents dip appearance, whereas the addition  after heating is without effect.	transcription
53895	17	335165	5	NULL	NULL	0	NULL	statement 17			prevents					dip appearance					NULL	PS II membranes	0	NULL	NULL	NULL	abs-batch0530-0539_photosynth-res_65_1_16228469_s_6	16228469	Presence of stabilizing cosolutes (glycine  betaine, sucrose) or addition of donor-side cofactors (bicarbonate, chloride,  calcium) to PS II membranes before heating (47 degrees C, 5 min) diminishes  J-P phase suppression and prevents dip appearance, whereas the addition  after heating is without effect.	transcription
53896	18	335165	5	NULL	NULL	0	NULL	calcium		addition of	diminishes					J-P phase		suppression of			NULL	PS II membranes	0	NULL	NULL	NULL	abs-batch0530-0539_photosynth-res_65_1_16228469_s_6	16228469	Presence of stabilizing cosolutes (glycine  betaine, sucrose) or addition of donor-side cofactors (bicarbonate, chloride,  calcium) to PS II membranes before heating (47 degrees C, 5 min) diminishes  J-P phase suppression and prevents dip appearance, whereas the addition  after heating is without effect.	transcription
53897	19	335165	5	NULL	NULL	0	NULL	statement 18			occurs before					heating					NULL		0	NULL	NULL	NULL	abs-batch0530-0539_photosynth-res_65_1_16228469_s_6	16228469	Presence of stabilizing cosolutes (glycine  betaine, sucrose) or addition of donor-side cofactors (bicarbonate, chloride,  calcium) to PS II membranes before heating (47 degrees C, 5 min) diminishes  J-P phase suppression and prevents dip appearance, whereas the addition  after heating is without effect.	transcription
53898	20	335165	5	NULL	NULL	0	NULL	statement 18			prevents					dip appearance					NULL	PS II membranes	0	NULL	NULL	NULL	abs-batch0530-0539_photosynth-res_65_1_16228469_s_6	16228469	Presence of stabilizing cosolutes (glycine  betaine, sucrose) or addition of donor-side cofactors (bicarbonate, chloride,  calcium) to PS II membranes before heating (47 degrees C, 5 min) diminishes  J-P phase suppression and prevents dip appearance, whereas the addition  after heating is without effect.	transcription
53899	1	335166	5	NULL	NULL	0	NULL	FIB		human	interacts with			N-terminal glycine- and arginine-rich domain (residues 1-77)		SF2A-p32					NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_279_3_14583623_s_4	14583623	Here, we demonstrate that the human  FIB N-terminal glycine- and arginine-rich domain (residues 1-77) and its  spacer region 1 (78-132) interact with splicing factor 2-associated p32  (SF2A-p32) and that the FIB methyltransferase-like domain (133-321) interacts  with protein-arginine methyltransferase 5 (PRMT5, Janus kinase-binding  protein 1).	transcription
53900	2	335166	5	NULL	NULL	0	NULL	FIB		human	interacts with			spacer region 1 (78-132)		SF2A-p32					NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_279_3_14583623_s_4	14583623	Here, we demonstrate that the human  FIB N-terminal glycine- and arginine-rich domain (residues 1-77) and its  spacer region 1 (78-132) interact with splicing factor 2-associated p32  (SF2A-p32) and that the FIB methyltransferase-like domain (133-321) interacts  with protein-arginine methyltransferase 5 (PRMT5, Janus kinase-binding  protein 1).	transcription
53901	3	335166	5	NULL	NULL	0	NULL	FIB		human	interacts with			methyltransferase-like domain (133-321)		PRMT5					NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_279_3_14583623_s_4	14583623	Here, we demonstrate that the human  FIB N-terminal glycine- and arginine-rich domain (residues 1-77) and its  spacer region 1 (78-132) interact with splicing factor 2-associated p32  (SF2A-p32) and that the FIB methyltransferase-like domain (133-321) interacts  with protein-arginine methyltransferase 5 (PRMT5, Janus kinase-binding  protein 1).	transcription
53902	4	335166	5	NULL	NULL	0	NULL	SF2A-p32			is					splicing factor 2-associated p32					NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_279_3_14583623_s_4	14583623	Here, we demonstrate that the human  FIB N-terminal glycine- and arginine-rich domain (residues 1-77) and its  spacer region 1 (78-132) interact with splicing factor 2-associated p32  (SF2A-p32) and that the FIB methyltransferase-like domain (133-321) interacts  with protein-arginine methyltransferase 5 (PRMT5, Janus kinase-binding  protein 1).	transcription
53903	5	335166	5	NULL	NULL	0	NULL	PRMT5			is					protein-arginine methyltransferase 5					NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_279_3_14583623_s_4	14583623	Here, we demonstrate that the human  FIB N-terminal glycine- and arginine-rich domain (residues 1-77) and its  spacer region 1 (78-132) interact with splicing factor 2-associated p32  (SF2A-p32) and that the FIB methyltransferase-like domain (133-321) interacts  with protein-arginine methyltransferase 5 (PRMT5, Janus kinase-binding  protein 1).	transcription
53904	6	335166	5	NULL	NULL	0	NULL	PRMT5			is					Janus kinase-binding protein 1		synonym of			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_279_3_14583623_s_4	14583623	Here, we demonstrate that the human  FIB N-terminal glycine- and arginine-rich domain (residues 1-77) and its  spacer region 1 (78-132) interact with splicing factor 2-associated p32  (SF2A-p32) and that the FIB methyltransferase-like domain (133-321) interacts  with protein-arginine methyltransferase 5 (PRMT5, Janus kinase-binding  protein 1).	transcription
55206	1	335166	7	NULL	NULL	0	NULL	FIB		human	interacts with			N-terminal glycine rich domain (residues 1-77)		SF2A-p32					NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_279_3_14583623_s_4	14583623	Here, we demonstrate that the human  FIB N-terminal glycine- and arginine-rich domain (residues 1-77) and its  spacer region 1 (78-132) interact with splicing factor 2-associated p32  (SF2A-p32) and that the FIB methyltransferase-like domain (133-321) interacts  with protein-arginine methyltransferase 5 (PRMT5, Janus kinase-binding  protein 1).	transcription
55207	2	335166	7	NULL	NULL	0	NULL	FIB		human	interacts with			N-terminal arginine-rich domain (residues 1-77)		SF2A-p32					NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_279_3_14583623_s_4	14583623	Here, we demonstrate that the human  FIB N-terminal glycine- and arginine-rich domain (residues 1-77) and its  spacer region 1 (78-132) interact with splicing factor 2-associated p32  (SF2A-p32) and that the FIB methyltransferase-like domain (133-321) interacts  with protein-arginine methyltransferase 5 (PRMT5, Janus kinase-binding  protein 1).	transcription
55208	3	335166	7	NULL	NULL	0	NULL	FIB		human	interacts with			spacer region 1 (78-132)		SF2A-p32					NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_279_3_14583623_s_4	14583623	Here, we demonstrate that the human  FIB N-terminal glycine- and arginine-rich domain (residues 1-77) and its  spacer region 1 (78-132) interact with splicing factor 2-associated p32  (SF2A-p32) and that the FIB methyltransferase-like domain (133-321) interacts  with protein-arginine methyltransferase 5 (PRMT5, Janus kinase-binding  protein 1).	transcription
55209	4	335166	7	NULL	NULL	0	NULL	 FIB			interacts with			methyltransferase-like domain (133-321)		PRMT5					NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_279_3_14583623_s_4	14583623	Here, we demonstrate that the human  FIB N-terminal glycine- and arginine-rich domain (residues 1-77) and its  spacer region 1 (78-132) interact with splicing factor 2-associated p32  (SF2A-p32) and that the FIB methyltransferase-like domain (133-321) interacts  with protein-arginine methyltransferase 5 (PRMT5, Janus kinase-binding  protein 1).	transcription
55210	5	335166	7	NULL	NULL	0	NULL	FIB			interacts with			methyltransferase-like domain (133-321)		Janus kinase-binding protein 1					NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_279_3_14583623_s_4	14583623	Here, we demonstrate that the human  FIB N-terminal glycine- and arginine-rich domain (residues 1-77) and its  spacer region 1 (78-132) interact with splicing factor 2-associated p32  (SF2A-p32) and that the FIB methyltransferase-like domain (133-321) interacts  with protein-arginine methyltransferase 5 (PRMT5, Janus kinase-binding  protein 1).	transcription
55211	6	335166	7	NULL	NULL	0	NULL	SF2A-p32			is					splicing factor 2-associated p32					NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_279_3_14583623_s_4	14583623	Here, we demonstrate that the human  FIB N-terminal glycine- and arginine-rich domain (residues 1-77) and its  spacer region 1 (78-132) interact with splicing factor 2-associated p32  (SF2A-p32) and that the FIB methyltransferase-like domain (133-321) interacts  with protein-arginine methyltransferase 5 (PRMT5, Janus kinase-binding  protein 1).	transcription
55212	7	335166	7	NULL	NULL	0	NULL	PRMT5			is					protein-arginine methyltransferase 5					NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-biol-chem_279_3_14583623_s_4	14583623	Here, we demonstrate that the human  FIB N-terminal glycine- and arginine-rich domain (residues 1-77) and its  spacer region 1 (78-132) interact with splicing factor 2-associated p32  (SF2A-p32) and that the FIB methyltransferase-like domain (133-321) interacts  with protein-arginine methyltransferase 5 (PRMT5, Janus kinase-binding  protein 1).	transcription
53907	1	335167	5	NULL	NULL	0	NULL	GlyRs			is activated by					glycine					NULL		0	NULL	NULL	NULL	gw70_jneurophysiol_95_4_2366_s_160	16381810	In voltage-clamp recordings, we found that activation of GlyRs by bath application of glycine (300 muM; CsCl pipette solution) elicited a >50% depression of both EPSCs (68  plus-or-minus  15%  n = 5 pyramidal cells; 64  plus-or-minus  5%  n = 10 interneurons) and IPSCs (52  plus-or-minus  5%,  n = 5 pyramidal cells; 64  plus-or-minus  6%,  n = 7 interneurons) that quickly recovered after washout ( Fig. 4).	transcription
53908	2	335167	5	NULL	NULL	0	NULL	statement 1			elicits					EPSCs		depression of			NULL		0	NULL	NULL	NULL	gw70_jneurophysiol_95_4_2366_s_160	16381810	In voltage-clamp recordings, we found that activation of GlyRs by bath application of glycine (300 muM; CsCl pipette solution) elicited a >50% depression of both EPSCs (68  plus-or-minus  15%  n = 5 pyramidal cells; 64  plus-or-minus  5%  n = 10 interneurons) and IPSCs (52  plus-or-minus  5%,  n = 5 pyramidal cells; 64  plus-or-minus  6%,  n = 7 interneurons) that quickly recovered after washout ( Fig. 4).	transcription
53909	3	335167	5	NULL	NULL	0	NULL	statement 1			elicits					IPSCs		depression of			NULL		0	NULL	NULL	NULL	gw70_jneurophysiol_95_4_2366_s_160	16381810	In voltage-clamp recordings, we found that activation of GlyRs by bath application of glycine (300 muM; CsCl pipette solution) elicited a >50% depression of both EPSCs (68  plus-or-minus  15%  n = 5 pyramidal cells; 64  plus-or-minus  5%  n = 10 interneurons) and IPSCs (52  plus-or-minus  5%,  n = 5 pyramidal cells; 64  plus-or-minus  6%,  n = 7 interneurons) that quickly recovered after washout ( Fig. 4).	transcription
55213	1	335167	7	NULL	NULL	0	NULL	glycine			activates					GlyRs					NULL		0	NULL	NULL	NULL	gw70_jneurophysiol_95_4_2366_s_160	16381810	In voltage-clamp recordings, we found that activation of GlyRs by bath application of glycine (300 muM; CsCl pipette solution) elicited a >50% depression of both EPSCs (68  plus-or-minus  15%  n = 5 pyramidal cells; 64  plus-or-minus  5%  n = 10 interneurons) and IPSCs (52  plus-or-minus  5%,  n = 5 pyramidal cells; 64  plus-or-minus  6%,  n = 7 interneurons) that quickly recovered after washout ( Fig. 4).	transcription
55214	2	335167	7	NULL	NULL	0	NULL	statement 1			elicits					EPSCs		depression of			NULL		0	NULL	NULL	NULL	gw70_jneurophysiol_95_4_2366_s_160	16381810	In voltage-clamp recordings, we found that activation of GlyRs by bath application of glycine (300 muM; CsCl pipette solution) elicited a >50% depression of both EPSCs (68  plus-or-minus  15%  n = 5 pyramidal cells; 64  plus-or-minus  5%  n = 10 interneurons) and IPSCs (52  plus-or-minus  5%,  n = 5 pyramidal cells; 64  plus-or-minus  6%,  n = 7 interneurons) that quickly recovered after washout ( Fig. 4).	transcription
55215	3	335167	7	NULL	NULL	0	NULL	statement 1			elicits					IPSCs		depression of			NULL		0	NULL	NULL	NULL	gw70_jneurophysiol_95_4_2366_s_160	16381810	In voltage-clamp recordings, we found that activation of GlyRs by bath application of glycine (300 muM; CsCl pipette solution) elicited a >50% depression of both EPSCs (68  plus-or-minus  15%  n = 5 pyramidal cells; 64  plus-or-minus  5%  n = 10 interneurons) and IPSCs (52  plus-or-minus  5%,  n = 5 pyramidal cells; 64  plus-or-minus  6%,  n = 7 interneurons) that quickly recovered after washout ( Fig. 4).	transcription
53910	1	335174	5	NULL	NULL	0	NULL	DCS			is					D-cycloserine					NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_11_4011_s_127	10818136	C, D-cycloserine ( DCS), a partial agonist at the glycine site of the NMDA receptor enhanced at 1 mg/kg haloperidol (0.3 mg/kg)-mediated  c-fos induction (compare  H 0.3 with  DCS 1 H 0.3) but had no significant effect at 5 mg/kg (compare  H 0.3 with  DCS 5 H 0.3).	transcription
53911	2	335174	5	NULL	NULL	0	NULL	DCS			is an agonist of		partial			NMDA receptor			glycine site		NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_11_4011_s_127	10818136	C, D-cycloserine ( DCS), a partial agonist at the glycine site of the NMDA receptor enhanced at 1 mg/kg haloperidol (0.3 mg/kg)-mediated  c-fos induction (compare  H 0.3 with  DCS 1 H 0.3) but had no significant effect at 5 mg/kg (compare  H 0.3 with  DCS 5 H 0.3).	transcription
53912	3	335174	5	NULL	NULL	0	NULL	c-fos		induction of	is mediated by					haloperidol					NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_11_4011_s_127	10818136	C, D-cycloserine ( DCS), a partial agonist at the glycine site of the NMDA receptor enhanced at 1 mg/kg haloperidol (0.3 mg/kg)-mediated  c-fos induction (compare  H 0.3 with  DCS 1 H 0.3) but had no significant effect at 5 mg/kg (compare  H 0.3 with  DCS 5 H 0.3).	transcription
53913	4	335174	5	NULL	NULL	0	NULL	DCS			enhance					statement 3					NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_11_4011_s_127	10818136	C, D-cycloserine ( DCS), a partial agonist at the glycine site of the NMDA receptor enhanced at 1 mg/kg haloperidol (0.3 mg/kg)-mediated  c-fos induction (compare  H 0.3 with  DCS 1 H 0.3) but had no significant effect at 5 mg/kg (compare  H 0.3 with  DCS 5 H 0.3).	transcription
55216	1	335174	7	NULL	NULL	0	NULL	DCS			agonist of		partial			NMDA receptor			glycine site of		NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_11_4011_s_127	10818136	C, D-cycloserine ( DCS), a partial agonist at the glycine site of the NMDA receptor enhanced at 1 mg/kg haloperidol (0.3 mg/kg)-mediated  c-fos induction (compare  H 0.3 with  DCS 1 H 0.3) but had no significant effect at 5 mg/kg (compare  H 0.3 with  DCS 5 H 0.3).	transcription
55217	2	335174	7	NULL	NULL	0	NULL	haloperidol			mediates					c-fos		induction of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_11_4011_s_127	10818136	C, D-cycloserine ( DCS), a partial agonist at the glycine site of the NMDA receptor enhanced at 1 mg/kg haloperidol (0.3 mg/kg)-mediated  c-fos induction (compare  H 0.3 with  DCS 1 H 0.3) but had no significant effect at 5 mg/kg (compare  H 0.3 with  DCS 5 H 0.3).	transcription
55218	3	335174	7	NULL	NULL	0	NULL	statement 1			enhanced upon					statement 2					NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_11_4011_s_127	10818136	C, D-cycloserine ( DCS), a partial agonist at the glycine site of the NMDA receptor enhanced at 1 mg/kg haloperidol (0.3 mg/kg)-mediated  c-fos induction (compare  H 0.3 with  DCS 1 H 0.3) but had no significant effect at 5 mg/kg (compare  H 0.3 with  DCS 5 H 0.3).	transcription
55219	4	335174	7	NULL	NULL	0	NULL	DCS			is					D-cycloserine					NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_11_4011_s_127	10818136	C, D-cycloserine ( DCS), a partial agonist at the glycine site of the NMDA receptor enhanced at 1 mg/kg haloperidol (0.3 mg/kg)-mediated  c-fos induction (compare  H 0.3 with  DCS 1 H 0.3) but had no significant effect at 5 mg/kg (compare  H 0.3 with  DCS 5 H 0.3).	transcription
53916	1	335179	5	NULL	NULL	0	NULL	D,L-APV			block					NMDA receptors		potential activation of			NULL		0	NULL	NULL	NULL	gw70_jneurophysiol_95_4_2366_s_273	16381810	When D,L-APV (100 muM) was included in the bath solution to block potential activation of  NMDA receptors by increased local glycine concentrations during GlyT1 blockade with  NFPS, the percentage of trials that elicited suprathreshold EPSPs was still not significantly  decreased compared with control (without D-APV; 5  plus-or-minus  4%,  n = 4,  P > 0.05, data not shown).	transcription
53917	2	335179	5	NULL	NULL	0	NULL	NFPS			block					GlyT1					NULL		0	NULL	NULL	NULL	gw70_jneurophysiol_95_4_2366_s_273	16381810	When D,L-APV (100 muM) was included in the bath solution to block potential activation of  NMDA receptors by increased local glycine concentrations during GlyT1 blockade with  NFPS, the percentage of trials that elicited suprathreshold EPSPs was still not significantly  decreased compared with control (without D-APV; 5  plus-or-minus  4%,  n = 4,  P > 0.05, data not shown).	transcription
53918	3	335179	5	NULL	NULL	0	NULL	statement 2			results in					glycine		increase in;;concentration of;;local			NULL		0	NULL	NULL	NULL	gw70_jneurophysiol_95_4_2366_s_273	16381810	When D,L-APV (100 muM) was included in the bath solution to block potential activation of  NMDA receptors by increased local glycine concentrations during GlyT1 blockade with  NFPS, the percentage of trials that elicited suprathreshold EPSPs was still not significantly  decreased compared with control (without D-APV; 5  plus-or-minus  4%,  n = 4,  P > 0.05, data not shown).	transcription
53919	4	335179	5	NULL	NULL	0	NULL	statement 3			leads to					statement 1					NULL		0	NULL	NULL	NULL	gw70_jneurophysiol_95_4_2366_s_273	16381810	When D,L-APV (100 muM) was included in the bath solution to block potential activation of  NMDA receptors by increased local glycine concentrations during GlyT1 blockade with  NFPS, the percentage of trials that elicited suprathreshold EPSPs was still not significantly  decreased compared with control (without D-APV; 5  plus-or-minus  4%,  n = 4,  P > 0.05, data not shown).	transcription
55355	1	335179	7	NULL	NULL	0	NULL	D,L-APV			block					NMDA receptor		potential activation of			NULL		0	NULL	NULL	NULL	gw70_jneurophysiol_95_4_2366_s_273	16381810	When D,L-APV (100 muM) was included in the bath solution to block potential activation of  NMDA receptors by increased local glycine concentrations during GlyT1 blockade with  NFPS, the percentage of trials that elicited suprathreshold EPSPs was still not significantly  decreased compared with control (without D-APV; 5  plus-or-minus  4%,  n = 4,  P > 0.05, data not shown).	transcription
55363	2	335179	7	NULL	NULL	0	NULL	statement 1			occur by					glycine		increased concentration of			NULL		0	NULL	NULL	NULL	gw70_jneurophysiol_95_4_2366_s_273	16381810	When D,L-APV (100 muM) was included in the bath solution to block potential activation of  NMDA receptors by increased local glycine concentrations during GlyT1 blockade with  NFPS, the percentage of trials that elicited suprathreshold EPSPs was still not significantly  decreased compared with control (without D-APV; 5  plus-or-minus  4%,  n = 4,  P > 0.05, data not shown).	transcription
55365	3	335179	7	NULL	NULL	0	NULL	NFPS			blocks					GlyT1					NULL		0	NULL	NULL	NULL	gw70_jneurophysiol_95_4_2366_s_273	16381810	When D,L-APV (100 muM) was included in the bath solution to block potential activation of  NMDA receptors by increased local glycine concentrations during GlyT1 blockade with  NFPS, the percentage of trials that elicited suprathreshold EPSPs was still not significantly  decreased compared with control (without D-APV; 5  plus-or-minus  4%,  n = 4,  P > 0.05, data not shown).	transcription
55367	4	335179	7	NULL	NULL	0	NULL	statement 1			occur during					statement 3					NULL		0	NULL	NULL	NULL	gw70_jneurophysiol_95_4_2366_s_273	16381810	When D,L-APV (100 muM) was included in the bath solution to block potential activation of  NMDA receptors by increased local glycine concentrations during GlyT1 blockade with  NFPS, the percentage of trials that elicited suprathreshold EPSPs was still not significantly  decreased compared with control (without D-APV; 5  plus-or-minus  4%,  n = 4,  P > 0.05, data not shown).	transcription
53924	1	335180	5	NULL	NULL	0	NULL	glycine			effects					VZ cells					NULL		0	NULL	NULL	NULL	gw70_pnas_102_52_19174_s_195	16357207	Most important, the effect of glycine on VZ cells is blocked by TTX (9.0  plus-or-minus  1.4%;  P < 0.05;  n = 5; data not shown), indicating that GlyR activation is sufficient to trigger both the activation of PP cells that express Na+ channels and the propagation of the Ca2+ signal to other cells in a manner that is similar to that observed with direct activation of the Na+ channels with veratridine.	transcription
53925	2	335180	5	NULL	NULL	0	NULL	TTX			blocks					statement 1					NULL		0	NULL	NULL	NULL	gw70_pnas_102_52_19174_s_195	16357207	Most important, the effect of glycine on VZ cells is blocked by TTX (9.0  plus-or-minus  1.4%;  P < 0.05;  n = 5; data not shown), indicating that GlyR activation is sufficient to trigger both the activation of PP cells that express Na+ channels and the propagation of the Ca2+ signal to other cells in a manner that is similar to that observed with direct activation of the Na+ channels with veratridine.	transcription
53926	3	335180	5	NULL	NULL	0	NULL	PP cells			express					Na+ channels					NULL		0	NULL	NULL	NULL	gw70_pnas_102_52_19174_s_195	16357207	Most important, the effect of glycine on VZ cells is blocked by TTX (9.0  plus-or-minus  1.4%;  P < 0.05;  n = 5; data not shown), indicating that GlyR activation is sufficient to trigger both the activation of PP cells that express Na+ channels and the propagation of the Ca2+ signal to other cells in a manner that is similar to that observed with direct activation of the Na+ channels with veratridine.	transcription
53927	4	335180	5	NULL	NULL	0	NULL	GlyR		activation of	triggers					statement 3		activation of			NULL		0	NULL	NULL	NULL	gw70_pnas_102_52_19174_s_195	16357207	Most important, the effect of glycine on VZ cells is blocked by TTX (9.0  plus-or-minus  1.4%;  P < 0.05;  n = 5; data not shown), indicating that GlyR activation is sufficient to trigger both the activation of PP cells that express Na+ channels and the propagation of the Ca2+ signal to other cells in a manner that is similar to that observed with direct activation of the Na+ channels with veratridine.	transcription
53928	5	335180	5	NULL	NULL	0	NULL	Ca2+ signal			is propagated to					cells					NULL		0	NULL	NULL	NULL	gw70_pnas_102_52_19174_s_195	16357207	Most important, the effect of glycine on VZ cells is blocked by TTX (9.0  plus-or-minus  1.4%;  P < 0.05;  n = 5; data not shown), indicating that GlyR activation is sufficient to trigger both the activation of PP cells that express Na+ channels and the propagation of the Ca2+ signal to other cells in a manner that is similar to that observed with direct activation of the Na+ channels with veratridine.	transcription
53929	6	335180	5	NULL	NULL	0	NULL	GlyR		activation of	triggers					statement 6					NULL		0	NULL	NULL	NULL	gw70_pnas_102_52_19174_s_195	16357207	Most important, the effect of glycine on VZ cells is blocked by TTX (9.0  plus-or-minus  1.4%;  P < 0.05;  n = 5; data not shown), indicating that GlyR activation is sufficient to trigger both the activation of PP cells that express Na+ channels and the propagation of the Ca2+ signal to other cells in a manner that is similar to that observed with direct activation of the Na+ channels with veratridine.	transcription
53930	7	335180	5	NULL	NULL	0	NULL	veratridine			activates		directly			Na+ channels					NULL		0	NULL	NULL	NULL	gw70_pnas_102_52_19174_s_195	16357207	Most important, the effect of glycine on VZ cells is blocked by TTX (9.0  plus-or-minus  1.4%;  P < 0.05;  n = 5; data not shown), indicating that GlyR activation is sufficient to trigger both the activation of PP cells that express Na+ channels and the propagation of the Ca2+ signal to other cells in a manner that is similar to that observed with direct activation of the Na+ channels with veratridine.	transcription
55370	1	335180	7	NULL	NULL	0	NULL	TTX			blocks					glycine		effect of			NULL	VZ cells	0	NULL	NULL	NULL	gw70_pnas_102_52_19174_s_195	16357207	Most important, the effect of glycine on VZ cells is blocked by TTX (9.0  plus-or-minus  1.4%;  P < 0.05;  n = 5; data not shown), indicating that GlyR activation is sufficient to trigger both the activation of PP cells that express Na+ channels and the propagation of the Ca2+ signal to other cells in a manner that is similar to that observed with direct activation of the Na+ channels with veratridine.	transcription
55371	2	335180	7	NULL	NULL	0	NULL	PP cells			express					Na+ channels					NULL		0	NULL	NULL	NULL	gw70_pnas_102_52_19174_s_195	16357207	Most important, the effect of glycine on VZ cells is blocked by TTX (9.0  plus-or-minus  1.4%;  P < 0.05;  n = 5; data not shown), indicating that GlyR activation is sufficient to trigger both the activation of PP cells that express Na+ channels and the propagation of the Ca2+ signal to other cells in a manner that is similar to that observed with direct activation of the Na+ channels with veratridine.	transcription
55372	3	335180	7	NULL	NULL	0	NULL	GlyR		activation of	trigger					statement 2					NULL		0	NULL	NULL	NULL	gw70_pnas_102_52_19174_s_195	16357207	Most important, the effect of glycine on VZ cells is blocked by TTX (9.0  plus-or-minus  1.4%;  P < 0.05;  n = 5; data not shown), indicating that GlyR activation is sufficient to trigger both the activation of PP cells that express Na+ channels and the propagation of the Ca2+ signal to other cells in a manner that is similar to that observed with direct activation of the Na+ channels with veratridine.	transcription
55376	4	335180	7	NULL	NULL	0	NULL	GlyR		activation of	trigger					Ca2+ signal		propogation of			NULL		0	NULL	NULL	NULL	gw70_pnas_102_52_19174_s_195	16357207	Most important, the effect of glycine on VZ cells is blocked by TTX (9.0  plus-or-minus  1.4%;  P < 0.05;  n = 5; data not shown), indicating that GlyR activation is sufficient to trigger both the activation of PP cells that express Na+ channels and the propagation of the Ca2+ signal to other cells in a manner that is similar to that observed with direct activation of the Na+ channels with veratridine.	transcription
55382	5	335180	7	NULL	NULL	0	NULL	veratridine			activates		directly			Na+ channels					NULL		0	NULL	NULL	NULL	gw70_pnas_102_52_19174_s_195	16357207	Most important, the effect of glycine on VZ cells is blocked by TTX (9.0  plus-or-minus  1.4%;  P < 0.05;  n = 5; data not shown), indicating that GlyR activation is sufficient to trigger both the activation of PP cells that express Na+ channels and the propagation of the Ca2+ signal to other cells in a manner that is similar to that observed with direct activation of the Na+ channels with veratridine.	transcription
53937	1	335189	5	NULL	NULL	0	NULL	Propofol			induce					GABA currents		enhancement of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_20_17438_s_112	11877425	Mutation of TM1 Glycine on alpha1 and beta2 Subunit Diminishes Propofol-induced Enhancement of GABA Currents-- The modulating effect of propofol on currents induced by GABA at EC20 in the wild type and mutant receptors is summarized in Table  II, which shows the effect of the highest propofol concentration tested for each receptor combination without inducing direct activation: 50 muM for the alpha1beta2gamma2 and alpha1(G223F)beta2gamma2 and 5 muM for the alpha1beta2(G219F)gamma2 combinations.	transcription
53938	2	335189	5	NULL	NULL	0	NULL	TM1 Glycine			is mutated in								alpha1 subunit		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_20_17438_s_112	11877425	Mutation of TM1 Glycine on alpha1 and beta2 Subunit Diminishes Propofol-induced Enhancement of GABA Currents-- The modulating effect of propofol on currents induced by GABA at EC20 in the wild type and mutant receptors is summarized in Table  II, which shows the effect of the highest propofol concentration tested for each receptor combination without inducing direct activation: 50 muM for the alpha1beta2gamma2 and alpha1(G223F)beta2gamma2 and 5 muM for the alpha1beta2(G219F)gamma2 combinations.	transcription
53939	3	335189	5	NULL	NULL	0	NULL	TM1 Glycine			is mutated in								beta2 subunit		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_20_17438_s_112	11877425	Mutation of TM1 Glycine on alpha1 and beta2 Subunit Diminishes Propofol-induced Enhancement of GABA Currents-- The modulating effect of propofol on currents induced by GABA at EC20 in the wild type and mutant receptors is summarized in Table  II, which shows the effect of the highest propofol concentration tested for each receptor combination without inducing direct activation: 50 muM for the alpha1beta2gamma2 and alpha1(G223F)beta2gamma2 and 5 muM for the alpha1beta2(G219F)gamma2 combinations.	transcription
53940	4	335189	5	NULL	NULL	0	NULL	statement 2			diminishes					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_20_17438_s_112	11877425	Mutation of TM1 Glycine on alpha1 and beta2 Subunit Diminishes Propofol-induced Enhancement of GABA Currents-- The modulating effect of propofol on currents induced by GABA at EC20 in the wild type and mutant receptors is summarized in Table  II, which shows the effect of the highest propofol concentration tested for each receptor combination without inducing direct activation: 50 muM for the alpha1beta2gamma2 and alpha1(G223F)beta2gamma2 and 5 muM for the alpha1beta2(G219F)gamma2 combinations.	transcription
53941	5	335189	5	NULL	NULL	0	NULL	statement 3			diminishes					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_20_17438_s_112	11877425	Mutation of TM1 Glycine on alpha1 and beta2 Subunit Diminishes Propofol-induced Enhancement of GABA Currents-- The modulating effect of propofol on currents induced by GABA at EC20 in the wild type and mutant receptors is summarized in Table  II, which shows the effect of the highest propofol concentration tested for each receptor combination without inducing direct activation: 50 muM for the alpha1beta2gamma2 and alpha1(G223F)beta2gamma2 and 5 muM for the alpha1beta2(G219F)gamma2 combinations.	transcription
55390	1	335189	7	NULL	NULL	0	NULL	 Propofol			induce					GABA currents		enhancement of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_20_17438_s_112	11877425	Mutation of TM1 Glycine on alpha1 and beta2 Subunit Diminishes Propofol-induced Enhancement of GABA Currents-- The modulating effect of propofol on currents induced by GABA at EC20 in the wild type and mutant receptors is summarized in Table  II, which shows the effect of the highest propofol concentration tested for each receptor combination without inducing direct activation: 50 muM for the alpha1beta2gamma2 and alpha1(G223F)beta2gamma2 and 5 muM for the alpha1beta2(G219F)gamma2 combinations.	transcription
55483	2	335189	7	NULL	NULL	0	NULL	TM1		mutation of	diminishes			Glycine on alpha1 subunit		statement 1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_20_17438_s_112	11877425	Mutation of TM1 Glycine on alpha1 and beta2 Subunit Diminishes Propofol-induced Enhancement of GABA Currents-- The modulating effect of propofol on currents induced by GABA at EC20 in the wild type and mutant receptors is summarized in Table  II, which shows the effect of the highest propofol concentration tested for each receptor combination without inducing direct activation: 50 muM for the alpha1beta2gamma2 and alpha1(G223F)beta2gamma2 and 5 muM for the alpha1beta2(G219F)gamma2 combinations.	transcription
55484	3	335189	7	NULL	NULL	0	NULL	TM1		mutation of	diminishes			Glycine beta2 subunit		statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_20_17438_s_112	11877425	Mutation of TM1 Glycine on alpha1 and beta2 Subunit Diminishes Propofol-induced Enhancement of GABA Currents-- The modulating effect of propofol on currents induced by GABA at EC20 in the wild type and mutant receptors is summarized in Table  II, which shows the effect of the highest propofol concentration tested for each receptor combination without inducing direct activation: 50 muM for the alpha1beta2gamma2 and alpha1(G223F)beta2gamma2 and 5 muM for the alpha1beta2(G219F)gamma2 combinations.	transcription
53942	1	335191	5	NULL	NULL	0	NULL	p53		MT	activates					MDR1				promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_39359_s_114	11483599	We found that although other MT p53s activated the  MDR1 promoter (see Fig.  5), the p53 aspartate to glycine 281 MT (p53-281) was the most potent activator of  MDR1 and that transcriptional activation required an intact transactivation domain because p53-281 containing mutations at amino acids 14 and 19 was ineffective in up-regulating the  MDR1 promoter (Fig.  2 A).	transcription
53943	2	335191	5	NULL	NULL	0	NULL	p53-281		MT	is					p53 aspartate to glycine 281					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_39359_s_114	11483599	We found that although other MT p53s activated the  MDR1 promoter (see Fig.  5), the p53 aspartate to glycine 281 MT (p53-281) was the most potent activator of  MDR1 and that transcriptional activation required an intact transactivation domain because p53-281 containing mutations at amino acids 14 and 19 was ineffective in up-regulating the  MDR1 promoter (Fig.  2 A).	transcription
53944	3	335191	5	NULL	NULL	0	NULL	p53-281		MT	activates		potent			MDR1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_39359_s_114	11483599	We found that although other MT p53s activated the  MDR1 promoter (see Fig.  5), the p53 aspartate to glycine 281 MT (p53-281) was the most potent activator of  MDR1 and that transcriptional activation required an intact transactivation domain because p53-281 containing mutations at amino acids 14 and 19 was ineffective in up-regulating the  MDR1 promoter (Fig.  2 A).	transcription
53945	4	335191	5	NULL	NULL	0	NULL	p53-281			conatins							mutation of	amino acids 14 and 19		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_39359_s_114	11483599	We found that although other MT p53s activated the  MDR1 promoter (see Fig.  5), the p53 aspartate to glycine 281 MT (p53-281) was the most potent activator of  MDR1 and that transcriptional activation required an intact transactivation domain because p53-281 containing mutations at amino acids 14 and 19 was ineffective in up-regulating the  MDR1 promoter (Fig.  2 A).	transcription
53946	5	335191	5	NULL	NULL	0	NULL	statement 1			does not upregulate					MDR1				promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_39359_s_114	11483599	We found that although other MT p53s activated the  MDR1 promoter (see Fig.  5), the p53 aspartate to glycine 281 MT (p53-281) was the most potent activator of  MDR1 and that transcriptional activation required an intact transactivation domain because p53-281 containing mutations at amino acids 14 and 19 was ineffective in up-regulating the  MDR1 promoter (Fig.  2 A).	transcription
53947	6	335191	5	NULL	NULL	0	NULL	transcription		activation of	requires							intact	 transactivation domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_39359_s_114	11483599	We found that although other MT p53s activated the  MDR1 promoter (see Fig.  5), the p53 aspartate to glycine 281 MT (p53-281) was the most potent activator of  MDR1 and that transcriptional activation required an intact transactivation domain because p53-281 containing mutations at amino acids 14 and 19 was ineffective in up-regulating the  MDR1 promoter (Fig.  2 A).	transcription
55485	1	335191	7	NULL	NULL	0	NULL	p53		MT	activate					MDR1				promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_39359_s_114	11483599	We found that although other MT p53s activated the  MDR1 promoter (see Fig.  5), the p53 aspartate to glycine 281 MT (p53-281) was the most potent activator of  MDR1 and that transcriptional activation required an intact transactivation domain because p53-281 containing mutations at amino acids 14 and 19 was ineffective in up-regulating the  MDR1 promoter (Fig.  2 A).	transcription
55486	2	335191	7	NULL	NULL	0	NULL	p53		MT	activate		potently	aspartate to glycine 281		MDR1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_39359_s_114	11483599	We found that although other MT p53s activated the  MDR1 promoter (see Fig.  5), the p53 aspartate to glycine 281 MT (p53-281) was the most potent activator of  MDR1 and that transcriptional activation required an intact transactivation domain because p53-281 containing mutations at amino acids 14 and 19 was ineffective in up-regulating the  MDR1 promoter (Fig.  2 A).	transcription
55487	3	335191	7	NULL	NULL	0	NULL	p53-281			is					p53		MT	aspartate to glycine 281		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_39359_s_114	11483599	We found that although other MT p53s activated the  MDR1 promoter (see Fig.  5), the p53 aspartate to glycine 281 MT (p53-281) was the most potent activator of  MDR1 and that transcriptional activation required an intact transactivation domain because p53-281 containing mutations at amino acids 14 and 19 was ineffective in up-regulating the  MDR1 promoter (Fig.  2 A).	transcription
55488	4	335191	7	NULL	NULL	0	NULL	statement 2			require							intact	transactivation domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_39359_s_114	11483599	We found that although other MT p53s activated the  MDR1 promoter (see Fig.  5), the p53 aspartate to glycine 281 MT (p53-281) was the most potent activator of  MDR1 and that transcriptional activation required an intact transactivation domain because p53-281 containing mutations at amino acids 14 and 19 was ineffective in up-regulating the  MDR1 promoter (Fig.  2 A).	transcription
55489	5	335191	7	NULL	NULL	0	NULL	p53-281 		MT	does not upregulate			mutations at amino acids 14 and 19		MDR1				promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_39359_s_114	11483599	We found that although other MT p53s activated the  MDR1 promoter (see Fig.  5), the p53 aspartate to glycine 281 MT (p53-281) was the most potent activator of  MDR1 and that transcriptional activation required an intact transactivation domain because p53-281 containing mutations at amino acids 14 and 19 was ineffective in up-regulating the  MDR1 promoter (Fig.  2 A).	transcription
53948	1	335196	5	NULL	NULL	0	NULL	dGK/dAK			is associated with			glycine- and arginine-rich motifs		nucleotide-binding proteins			ATP-binding site		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_12_6602_s_21	7896799	Scanning for homology with structural  elements shown to be related to function in other kinases reveals that  dGK/dAK contains the glycine- and arginine-rich motifs associated with  the ATP- or GTP-binding sites of many nucleotide-binding proteins ( 9,  10) and which are also highly conserved in the  adenylate kinases ( 11) and herpesviral thymidine kinases (HSV  sites 1 and 5)( 12,  13) .	transcription
53949	2	335196	5	NULL	NULL	0	NULL	dGK/dAK			is associated with			glycine- and arginine-rich motifs		nucleotide-binding proteins			GTP-binding sites		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_12_6602_s_21	7896799	Scanning for homology with structural  elements shown to be related to function in other kinases reveals that  dGK/dAK contains the glycine- and arginine-rich motifs associated with  the ATP- or GTP-binding sites of many nucleotide-binding proteins ( 9,  10) and which are also highly conserved in the  adenylate kinases ( 11) and herpesviral thymidine kinases (HSV  sites 1 and 5)( 12,  13) .	transcription
53950	3	335196	5	NULL	NULL	0	NULL	dGK/dAK			is conserved in		highly	glycine- and arginine-rich motifs		adenylate kinases					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_12_6602_s_21	7896799	Scanning for homology with structural  elements shown to be related to function in other kinases reveals that  dGK/dAK contains the glycine- and arginine-rich motifs associated with  the ATP- or GTP-binding sites of many nucleotide-binding proteins ( 9,  10) and which are also highly conserved in the  adenylate kinases ( 11) and herpesviral thymidine kinases (HSV  sites 1 and 5)( 12,  13) .	transcription
53951	4	335196	5	NULL	NULL	0	NULL	dGK/dAK			is conserved in			glycine- and arginine-rich motifs		herpesviral thymidine kinases					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_12_6602_s_21	7896799	Scanning for homology with structural  elements shown to be related to function in other kinases reveals that  dGK/dAK contains the glycine- and arginine-rich motifs associated with  the ATP- or GTP-binding sites of many nucleotide-binding proteins ( 9,  10) and which are also highly conserved in the  adenylate kinases ( 11) and herpesviral thymidine kinases (HSV  sites 1 and 5)( 12,  13) .	transcription
55490	1	335196	7	NULL	NULL	0	NULL	dGK			contains								glycine rich motifs		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_12_6602_s_21	7896799	Scanning for homology with structural  elements shown to be related to function in other kinases reveals that  dGK/dAK contains the glycine- and arginine-rich motifs associated with  the ATP- or GTP-binding sites of many nucleotide-binding proteins ( 9,  10) and which are also highly conserved in the  adenylate kinases ( 11) and herpesviral thymidine kinases (HSV  sites 1 and 5)( 12,  13) .	transcription
55491	2	335196	7	NULL	NULL	0	NULL	dAK			contains								arginine-rich motifs		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_12_6602_s_21	7896799	Scanning for homology with structural  elements shown to be related to function in other kinases reveals that  dGK/dAK contains the glycine- and arginine-rich motifs associated with  the ATP- or GTP-binding sites of many nucleotide-binding proteins ( 9,  10) and which are also highly conserved in the  adenylate kinases ( 11) and herpesviral thymidine kinases (HSV  sites 1 and 5)( 12,  13) .	transcription
55492	3	335196	7	NULL	NULL	0	NULL	statement 1			associated with					nucleotide-binding proteins			ATP-binding site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_12_6602_s_21	7896799	Scanning for homology with structural  elements shown to be related to function in other kinases reveals that  dGK/dAK contains the glycine- and arginine-rich motifs associated with  the ATP- or GTP-binding sites of many nucleotide-binding proteins ( 9,  10) and which are also highly conserved in the  adenylate kinases ( 11) and herpesviral thymidine kinases (HSV  sites 1 and 5)( 12,  13) .	transcription
55493	4	335196	7	NULL	NULL	0	NULL	statement 1			associated with					nucleotide-binding proteins			GTP-binding sites		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_12_6602_s_21	7896799	Scanning for homology with structural  elements shown to be related to function in other kinases reveals that  dGK/dAK contains the glycine- and arginine-rich motifs associated with  the ATP- or GTP-binding sites of many nucleotide-binding proteins ( 9,  10) and which are also highly conserved in the  adenylate kinases ( 11) and herpesviral thymidine kinases (HSV  sites 1 and 5)( 12,  13) .	transcription
55494	5	335196	7	NULL	NULL	0	NULL	statement 2			associated with					nucleotide-binding proteins			ATP-binding site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_12_6602_s_21	7896799	Scanning for homology with structural  elements shown to be related to function in other kinases reveals that  dGK/dAK contains the glycine- and arginine-rich motifs associated with  the ATP- or GTP-binding sites of many nucleotide-binding proteins ( 9,  10) and which are also highly conserved in the  adenylate kinases ( 11) and herpesviral thymidine kinases (HSV  sites 1 and 5)( 12,  13) .	transcription
55495	6	335196	7	NULL	NULL	0	NULL	statement 2			associated with					nucleotide-binding proteins			GTP-binding sites		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_12_6602_s_21	7896799	Scanning for homology with structural  elements shown to be related to function in other kinases reveals that  dGK/dAK contains the glycine- and arginine-rich motifs associated with  the ATP- or GTP-binding sites of many nucleotide-binding proteins ( 9,  10) and which are also highly conserved in the  adenylate kinases ( 11) and herpesviral thymidine kinases (HSV  sites 1 and 5)( 12,  13) .	transcription
55496	7	335196	7	NULL	NULL	0	NULL				is highly conserved in			glycine-rich motifs		adenylate kinases					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_12_6602_s_21	7896799	Scanning for homology with structural  elements shown to be related to function in other kinases reveals that  dGK/dAK contains the glycine- and arginine-rich motifs associated with  the ATP- or GTP-binding sites of many nucleotide-binding proteins ( 9,  10) and which are also highly conserved in the  adenylate kinases ( 11) and herpesviral thymidine kinases (HSV  sites 1 and 5)( 12,  13) .	transcription
55497	8	335196	7	NULL	NULL	0	NULL				is highly conserved in			arginine-rich motifs		adenylate kinases					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_12_6602_s_21	7896799	Scanning for homology with structural  elements shown to be related to function in other kinases reveals that  dGK/dAK contains the glycine- and arginine-rich motifs associated with  the ATP- or GTP-binding sites of many nucleotide-binding proteins ( 9,  10) and which are also highly conserved in the  adenylate kinases ( 11) and herpesviral thymidine kinases (HSV  sites 1 and 5)( 12,  13) .	transcription
55498	9	335196	7	NULL	NULL	0	NULL				is highly conserved in			glycine-rich motifs		thymidine kinases		herpesviral 	HSV sites 1		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_12_6602_s_21	7896799	Scanning for homology with structural  elements shown to be related to function in other kinases reveals that  dGK/dAK contains the glycine- and arginine-rich motifs associated with  the ATP- or GTP-binding sites of many nucleotide-binding proteins ( 9,  10) and which are also highly conserved in the  adenylate kinases ( 11) and herpesviral thymidine kinases (HSV  sites 1 and 5)( 12,  13) .	transcription
55499	10	335196	7	NULL	NULL	0	NULL				is highly conserved in			glycine-rich motifs		 thymidine kinases		herpesviral	HSV sites 5		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_12_6602_s_21	7896799	Scanning for homology with structural  elements shown to be related to function in other kinases reveals that  dGK/dAK contains the glycine- and arginine-rich motifs associated with  the ATP- or GTP-binding sites of many nucleotide-binding proteins ( 9,  10) and which are also highly conserved in the  adenylate kinases ( 11) and herpesviral thymidine kinases (HSV  sites 1 and 5)( 12,  13) .	transcription
55500	11	335196	7	NULL	NULL	0	NULL				is highly conserved in			arginine-rich motifs		 thymidine kinases		herpesviral	HSV sites 1		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_12_6602_s_21	7896799	Scanning for homology with structural  elements shown to be related to function in other kinases reveals that  dGK/dAK contains the glycine- and arginine-rich motifs associated with  the ATP- or GTP-binding sites of many nucleotide-binding proteins ( 9,  10) and which are also highly conserved in the  adenylate kinases ( 11) and herpesviral thymidine kinases (HSV  sites 1 and 5)( 12,  13) .	transcription
55501	12	335196	7	NULL	NULL	0	NULL				is highly conserved in			arginine-rich motifs		thymidine kinases		herpesviral	HSV sites 5		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_12_6602_s_21	7896799	Scanning for homology with structural  elements shown to be related to function in other kinases reveals that  dGK/dAK contains the glycine- and arginine-rich motifs associated with  the ATP- or GTP-binding sites of many nucleotide-binding proteins ( 9,  10) and which are also highly conserved in the  adenylate kinases ( 11) and herpesviral thymidine kinases (HSV  sites 1 and 5)( 12,  13) .	transcription
53952	1	335199	5	NULL	NULL	0	NULL	mecamylamine stereoisomers			inhibits		transiently			NMDA receptor		response of			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_297_2_646_s_145	11303054	As shown in Fig.  5, whereas both mecamylamine stereoisomers applied at a concentration of 100 muM could produce a transient inhibition of NMDA receptor responses to the coapplication of 10 muM glutamate + 10 muM glycine ( p < 0.001), this effect was reversible after a 5-min wash. NMDA receptor responses obtained in the presence of mecamylamine were also analyzed in terms of net charge.	transcription
55502	1	335199	7	NULL	NULL	0	NULL	mecamylamine stereoisomers			inhibits		transiently			NMDA receptor					NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_297_2_646_s_145	11303054	As shown in Fig.  5, whereas both mecamylamine stereoisomers applied at a concentration of 100 muM could produce a transient inhibition of NMDA receptor responses to the coapplication of 10 muM glutamate + 10 muM glycine ( p < 0.001), this effect was reversible after a 5-min wash. NMDA receptor responses obtained in the presence of mecamylamine were also analyzed in terms of net charge.	transcription
53953	1	335201	5	NULL	NULL	0	NULL	class II enzymes			cleaves		homolytically			adenosylcobalamin					NULL		0	NULL	NULL	NULL	gw60_structure_2_9_793_s_91	7812713	Class I enzymes (subunit composition   2  2) carry the stable tyrosyl radical on a component different from the substrate binding component  [11  , class II enzymes (subunit composition usually   ) can cleave adenosylcobalamin homolytically to produce a transient 5 -deoxyadenosyl radical   [18,3]  , and class III enzymes (subunit composition   2) carry a stable glycine radical  [4  .	transcription
53954	2	335201	5	NULL	NULL	0	NULL	statement 1			produce					5 -deoxyadenosyl radical		transient			NULL		0	NULL	NULL	NULL	gw60_structure_2_9_793_s_91	7812713	Class I enzymes (subunit composition   2  2) carry the stable tyrosyl radical on a component different from the substrate binding component  [11  , class II enzymes (subunit composition usually   ) can cleave adenosylcobalamin homolytically to produce a transient 5 -deoxyadenosyl radical   [18,3]  , and class III enzymes (subunit composition   2) carry a stable glycine radical  [4  .	transcription
55503	1	335201	7	NULL	NULL	0	NULL	Class I enzymes			carry							stable	tyrosyl radical 		NULL		0	NULL	NULL	NULL	gw60_structure_2_9_793_s_91	7812713	Class I enzymes (subunit composition   2  2) carry the stable tyrosyl radical on a component different from the substrate binding component  [11  , class II enzymes (subunit composition usually   ) can cleave adenosylcobalamin homolytically to produce a transient 5 -deoxyadenosyl radical   [18,3]  , and class III enzymes (subunit composition   2) carry a stable glycine radical  [4  .	transcription
55504	2	335201	7	NULL	NULL	0	NULL	class II enzymes			cleave		could;;homolytically			adenosylcobalamin					NULL		0	NULL	NULL	NULL	gw60_structure_2_9_793_s_91	7812713	Class I enzymes (subunit composition   2  2) carry the stable tyrosyl radical on a component different from the substrate binding component  [11  , class II enzymes (subunit composition usually   ) can cleave adenosylcobalamin homolytically to produce a transient 5 -deoxyadenosyl radical   [18,3]  , and class III enzymes (subunit composition   2) carry a stable glycine radical  [4  .	transcription
55505	3	335201	7	NULL	NULL	0	NULL	statement 2			produce		transiently			5 -deoxyadenosyl radical					NULL		0	NULL	NULL	NULL	gw60_structure_2_9_793_s_91	7812713	Class I enzymes (subunit composition   2  2) carry the stable tyrosyl radical on a component different from the substrate binding component  [11  , class II enzymes (subunit composition usually   ) can cleave adenosylcobalamin homolytically to produce a transient 5 -deoxyadenosyl radical   [18,3]  , and class III enzymes (subunit composition   2) carry a stable glycine radical  [4  .	transcription
55506	4	335201	7	NULL	NULL	0	NULL	class III enzymes			carry					glycine radical		stable			NULL		0	NULL	NULL	NULL	gw60_structure_2_9_793_s_91	7812713	Class I enzymes (subunit composition   2  2) carry the stable tyrosyl radical on a component different from the substrate binding component  [11  , class II enzymes (subunit composition usually   ) can cleave adenosylcobalamin homolytically to produce a transient 5 -deoxyadenosyl radical   [18,3]  , and class III enzymes (subunit composition   2) carry a stable glycine radical  [4  .	transcription
55507	5	335201	7	NULL	NULL	0	NULL	statement 1			is not present in								substrate binding component		NULL		0	NULL	NULL	NULL	gw60_structure_2_9_793_s_91	7812713	Class I enzymes (subunit composition   2  2) carry the stable tyrosyl radical on a component different from the substrate binding component  [11  , class II enzymes (subunit composition usually   ) can cleave adenosylcobalamin homolytically to produce a transient 5 -deoxyadenosyl radical   [18,3]  , and class III enzymes (subunit composition   2) carry a stable glycine radical  [4  .	transcription
53955	1	335202	5	NULL	NULL	0	NULL	IGF-1		stimulation of	maintains					C/EBP		low nuclear levels of			NULL		0	NULL	NULL	NULL	gw60_neuron_39_4_625_s_194	12925277	(a1) IGF-1 stimulation maintains low nuclear levels of C/EBP  (lane 2), but levels increase when growth factor support is removed (lane 1) or when L channel or CaMK activities are inhibited (lanes 3 and 4); nimodipine, 5  M; KN62, 10  M. Conversely, NMDA receptor activity increases the levels in a calcineurin-dependent manner: blocking NMDA receptors with 100  M APV reduces nuclear C/EBP  (lane 5), stimulation with 300  M NMDA + 1  M glycine increases it (lane 6), but when 1  M deltamethrin is coapplied, nuclear levels decline (lane 7).	transcription
53956	2	335202	5	NULL	NULL	0	NULL	C/EBP		nuclear levels of	increase upon					growth factor support		removal of			NULL		0	NULL	NULL	NULL	gw60_neuron_39_4_625_s_194	12925277	(a1) IGF-1 stimulation maintains low nuclear levels of C/EBP  (lane 2), but levels increase when growth factor support is removed (lane 1) or when L channel or CaMK activities are inhibited (lanes 3 and 4); nimodipine, 5  M; KN62, 10  M. Conversely, NMDA receptor activity increases the levels in a calcineurin-dependent manner: blocking NMDA receptors with 100  M APV reduces nuclear C/EBP  (lane 5), stimulation with 300  M NMDA + 1  M glycine increases it (lane 6), but when 1  M deltamethrin is coapplied, nuclear levels decline (lane 7).	transcription
53957	3	335202	5	NULL	NULL	0	NULL	L channel		inhibition of;;activity of	increases					C/EBP		nuclear levels of			NULL		0	NULL	NULL	NULL	gw60_neuron_39_4_625_s_194	12925277	(a1) IGF-1 stimulation maintains low nuclear levels of C/EBP  (lane 2), but levels increase when growth factor support is removed (lane 1) or when L channel or CaMK activities are inhibited (lanes 3 and 4); nimodipine, 5  M; KN62, 10  M. Conversely, NMDA receptor activity increases the levels in a calcineurin-dependent manner: blocking NMDA receptors with 100  M APV reduces nuclear C/EBP  (lane 5), stimulation with 300  M NMDA + 1  M glycine increases it (lane 6), but when 1  M deltamethrin is coapplied, nuclear levels decline (lane 7).	transcription
53958	4	335202	5	NULL	NULL	0	NULL	CaMK		inhibition of;;activity of	increases					C/EBP		nuclear levels of			NULL		0	NULL	NULL	NULL	gw60_neuron_39_4_625_s_194	12925277	(a1) IGF-1 stimulation maintains low nuclear levels of C/EBP  (lane 2), but levels increase when growth factor support is removed (lane 1) or when L channel or CaMK activities are inhibited (lanes 3 and 4); nimodipine, 5  M; KN62, 10  M. Conversely, NMDA receptor activity increases the levels in a calcineurin-dependent manner: blocking NMDA receptors with 100  M APV reduces nuclear C/EBP  (lane 5), stimulation with 300  M NMDA + 1  M glycine increases it (lane 6), but when 1  M deltamethrin is coapplied, nuclear levels decline (lane 7).	transcription
53959	5	335202	5	NULL	NULL	0	NULL	NMDA receptor		activity of	increases					C/EBP		nuclear levels of			NULL		0	NULL	NULL	NULL	gw60_neuron_39_4_625_s_194	12925277	(a1) IGF-1 stimulation maintains low nuclear levels of C/EBP  (lane 2), but levels increase when growth factor support is removed (lane 1) or when L channel or CaMK activities are inhibited (lanes 3 and 4); nimodipine, 5  M; KN62, 10  M. Conversely, NMDA receptor activity increases the levels in a calcineurin-dependent manner: blocking NMDA receptors with 100  M APV reduces nuclear C/EBP  (lane 5), stimulation with 300  M NMDA + 1  M glycine increases it (lane 6), but when 1  M deltamethrin is coapplied, nuclear levels decline (lane 7).	transcription
53960	6	335202	5	NULL	NULL	0	NULL	statement 5			is dependent on					calcineurin					NULL		0	NULL	NULL	NULL	gw60_neuron_39_4_625_s_194	12925277	(a1) IGF-1 stimulation maintains low nuclear levels of C/EBP  (lane 2), but levels increase when growth factor support is removed (lane 1) or when L channel or CaMK activities are inhibited (lanes 3 and 4); nimodipine, 5  M; KN62, 10  M. Conversely, NMDA receptor activity increases the levels in a calcineurin-dependent manner: blocking NMDA receptors with 100  M APV reduces nuclear C/EBP  (lane 5), stimulation with 300  M NMDA + 1  M glycine increases it (lane 6), but when 1  M deltamethrin is coapplied, nuclear levels decline (lane 7).	transcription
53961	7	335202	5	NULL	NULL	0	NULL	NMDA receptors			is blocked by					APV					NULL		0	NULL	NULL	NULL	gw60_neuron_39_4_625_s_194	12925277	(a1) IGF-1 stimulation maintains low nuclear levels of C/EBP  (lane 2), but levels increase when growth factor support is removed (lane 1) or when L channel or CaMK activities are inhibited (lanes 3 and 4); nimodipine, 5  M; KN62, 10  M. Conversely, NMDA receptor activity increases the levels in a calcineurin-dependent manner: blocking NMDA receptors with 100  M APV reduces nuclear C/EBP  (lane 5), stimulation with 300  M NMDA + 1  M glycine increases it (lane 6), but when 1  M deltamethrin is coapplied, nuclear levels decline (lane 7).	transcription
53962	8	335202	5	NULL	NULL	0	NULL	statement 7			reduces					C/EBP		nuclear levels of			NULL		NULL	NULL	NULL	NULL	gw60_neuron_39_4_625_s_194	12925277	(a1) IGF-1 stimulation maintains low nuclear levels of C/EBP  (lane 2), but levels increase when growth factor support is removed (lane 1) or when L channel or CaMK activities are inhibited (lanes 3 and 4); nimodipine, 5  M; KN62, 10  M. Conversely, NMDA receptor activity increases the levels in a calcineurin-dependent manner: blocking NMDA receptors with 100  M APV reduces nuclear C/EBP  (lane 5), stimulation with 300  M NMDA + 1  M glycine increases it (lane 6), but when 1  M deltamethrin is coapplied, nuclear levels decline (lane 7).	transcription
53963	9	335202	5	NULL	NULL	0	NULL	NMDA			stimulates					NMDA receptors					NULL		0	NULL	NULL	NULL	gw60_neuron_39_4_625_s_194	12925277	(a1) IGF-1 stimulation maintains low nuclear levels of C/EBP  (lane 2), but levels increase when growth factor support is removed (lane 1) or when L channel or CaMK activities are inhibited (lanes 3 and 4); nimodipine, 5  M; KN62, 10  M. Conversely, NMDA receptor activity increases the levels in a calcineurin-dependent manner: blocking NMDA receptors with 100  M APV reduces nuclear C/EBP  (lane 5), stimulation with 300  M NMDA + 1  M glycine increases it (lane 6), but when 1  M deltamethrin is coapplied, nuclear levels decline (lane 7).	transcription
53964	10	335202	5	NULL	NULL	0	NULL	glycine			stimulates					NMDA receptors					NULL		0	NULL	NULL	NULL	gw60_neuron_39_4_625_s_194	12925277	(a1) IGF-1 stimulation maintains low nuclear levels of C/EBP  (lane 2), but levels increase when growth factor support is removed (lane 1) or when L channel or CaMK activities are inhibited (lanes 3 and 4); nimodipine, 5  M; KN62, 10  M. Conversely, NMDA receptor activity increases the levels in a calcineurin-dependent manner: blocking NMDA receptors with 100  M APV reduces nuclear C/EBP  (lane 5), stimulation with 300  M NMDA + 1  M glycine increases it (lane 6), but when 1  M deltamethrin is coapplied, nuclear levels decline (lane 7).	transcription
53965	11	335202	5	NULL	NULL	0	NULL	statement 9			occurs along with					statement 10					NULL		0	NULL	NULL	NULL	gw60_neuron_39_4_625_s_194	12925277	(a1) IGF-1 stimulation maintains low nuclear levels of C/EBP  (lane 2), but levels increase when growth factor support is removed (lane 1) or when L channel or CaMK activities are inhibited (lanes 3 and 4); nimodipine, 5  M; KN62, 10  M. Conversely, NMDA receptor activity increases the levels in a calcineurin-dependent manner: blocking NMDA receptors with 100  M APV reduces nuclear C/EBP  (lane 5), stimulation with 300  M NMDA + 1  M glycine increases it (lane 6), but when 1  M deltamethrin is coapplied, nuclear levels decline (lane 7).	transcription
53966	12	335202	5	NULL	NULL	0	NULL	statement 11			increases					C/EBP		nuclear levels of			NULL		NULL	NULL	NULL	NULL	gw60_neuron_39_4_625_s_194	12925277	(a1) IGF-1 stimulation maintains low nuclear levels of C/EBP  (lane 2), but levels increase when growth factor support is removed (lane 1) or when L channel or CaMK activities are inhibited (lanes 3 and 4); nimodipine, 5  M; KN62, 10  M. Conversely, NMDA receptor activity increases the levels in a calcineurin-dependent manner: blocking NMDA receptors with 100  M APV reduces nuclear C/EBP  (lane 5), stimulation with 300  M NMDA + 1  M glycine increases it (lane 6), but when 1  M deltamethrin is coapplied, nuclear levels decline (lane 7).	transcription
53967	13	335202	5	NULL	NULL	0	NULL	deltamethrin			declines					C/EBP		nuclear levels of			NULL		0	NULL	NULL	NULL	gw60_neuron_39_4_625_s_194	12925277	(a1) IGF-1 stimulation maintains low nuclear levels of C/EBP  (lane 2), but levels increase when growth factor support is removed (lane 1) or when L channel or CaMK activities are inhibited (lanes 3 and 4); nimodipine, 5  M; KN62, 10  M. Conversely, NMDA receptor activity increases the levels in a calcineurin-dependent manner: blocking NMDA receptors with 100  M APV reduces nuclear C/EBP  (lane 5), stimulation with 300  M NMDA + 1  M glycine increases it (lane 6), but when 1  M deltamethrin is coapplied, nuclear levels decline (lane 7).	transcription
55514	1	335202	7	NULL	NULL	0	NULL	IGF-1 		stimulation of	maintains					C/EBP		 low nuclear levels of 			NULL		0	NULL	NULL	NULL	gw60_neuron_39_4_625_s_194	12925277	(a1) IGF-1 stimulation maintains low nuclear levels of C/EBP  (lane 2), but levels increase when growth factor support is removed (lane 1) or when L channel or CaMK activities are inhibited (lanes 3 and 4); nimodipine, 5  M; KN62, 10  M. Conversely, NMDA receptor activity increases the levels in a calcineurin-dependent manner: blocking NMDA receptors with 100  M APV reduces nuclear C/EBP  (lane 5), stimulation with 300  M NMDA + 1  M glycine increases it (lane 6), but when 1  M deltamethrin is coapplied, nuclear levels decline (lane 7).	transcription
55521	2	335202	7	NULL	NULL	0	NULL	L channel 		inhibition of	increase					C/EBP		nuclear levels of			NULL		NULL	NULL	NULL	NULL	gw60_neuron_39_4_625_s_194	12925277	(a1) IGF-1 stimulation maintains low nuclear levels of C/EBP  (lane 2), but levels increase when growth factor support is removed (lane 1) or when L channel or CaMK activities are inhibited (lanes 3 and 4); nimodipine, 5  M; KN62, 10  M. Conversely, NMDA receptor activity increases the levels in a calcineurin-dependent manner: blocking NMDA receptors with 100  M APV reduces nuclear C/EBP  (lane 5), stimulation with 300  M NMDA + 1  M glycine increases it (lane 6), but when 1  M deltamethrin is coapplied, nuclear levels decline (lane 7).	transcription
55522	3	335202	7	NULL	NULL	0	NULL	CaMK		inhibition of;;activities of	increase					C/EBP		nuclear levels of			NULL		0	NULL	NULL	NULL	gw60_neuron_39_4_625_s_194	12925277	(a1) IGF-1 stimulation maintains low nuclear levels of C/EBP  (lane 2), but levels increase when growth factor support is removed (lane 1) or when L channel or CaMK activities are inhibited (lanes 3 and 4); nimodipine, 5  M; KN62, 10  M. Conversely, NMDA receptor activity increases the levels in a calcineurin-dependent manner: blocking NMDA receptors with 100  M APV reduces nuclear C/EBP  (lane 5), stimulation with 300  M NMDA + 1  M glycine increases it (lane 6), but when 1  M deltamethrin is coapplied, nuclear levels decline (lane 7).	transcription
55523	4	335202	7	NULL	NULL	0	NULL	 APV 			blocks					NMDA receptor					NULL		0	NULL	NULL	NULL	gw60_neuron_39_4_625_s_194	12925277	(a1) IGF-1 stimulation maintains low nuclear levels of C/EBP  (lane 2), but levels increase when growth factor support is removed (lane 1) or when L channel or CaMK activities are inhibited (lanes 3 and 4); nimodipine, 5  M; KN62, 10  M. Conversely, NMDA receptor activity increases the levels in a calcineurin-dependent manner: blocking NMDA receptors with 100  M APV reduces nuclear C/EBP  (lane 5), stimulation with 300  M NMDA + 1  M glycine increases it (lane 6), but when 1  M deltamethrin is coapplied, nuclear levels decline (lane 7).	transcription
55524	5	335202	7	NULL	NULL	0	NULL	statement 4			reduce					C/EBP		nuclear			NULL		0	NULL	NULL	NULL	gw60_neuron_39_4_625_s_194	12925277	(a1) IGF-1 stimulation maintains low nuclear levels of C/EBP  (lane 2), but levels increase when growth factor support is removed (lane 1) or when L channel or CaMK activities are inhibited (lanes 3 and 4); nimodipine, 5  M; KN62, 10  M. Conversely, NMDA receptor activity increases the levels in a calcineurin-dependent manner: blocking NMDA receptors with 100  M APV reduces nuclear C/EBP  (lane 5), stimulation with 300  M NMDA + 1  M glycine increases it (lane 6), but when 1  M deltamethrin is coapplied, nuclear levels decline (lane 7).	transcription
55626	6	335202	7	NULL	NULL	0	NULL	NMDA receptor		activity of	increase					C/EBP		nuclear levels of			NULL		NULL	NULL	NULL	NULL	gw60_neuron_39_4_625_s_194	12925277	(a1) IGF-1 stimulation maintains low nuclear levels of C/EBP  (lane 2), but levels increase when growth factor support is removed (lane 1) or when L channel or CaMK activities are inhibited (lanes 3 and 4); nimodipine, 5  M; KN62, 10  M. Conversely, NMDA receptor activity increases the levels in a calcineurin-dependent manner: blocking NMDA receptors with 100  M APV reduces nuclear C/EBP  (lane 5), stimulation with 300  M NMDA + 1  M glycine increases it (lane 6), but when 1  M deltamethrin is coapplied, nuclear levels decline (lane 7).	transcription
55627	7	335202	7	NULL	NULL	0	NULL	statement 6			depends on					calcineurin					NULL		0	NULL	NULL	NULL	gw60_neuron_39_4_625_s_194	12925277	(a1) IGF-1 stimulation maintains low nuclear levels of C/EBP  (lane 2), but levels increase when growth factor support is removed (lane 1) or when L channel or CaMK activities are inhibited (lanes 3 and 4); nimodipine, 5  M; KN62, 10  M. Conversely, NMDA receptor activity increases the levels in a calcineurin-dependent manner: blocking NMDA receptors with 100  M APV reduces nuclear C/EBP  (lane 5), stimulation with 300  M NMDA + 1  M glycine increases it (lane 6), but when 1  M deltamethrin is coapplied, nuclear levels decline (lane 7).	transcription
55628	8	335202	7	NULL	NULL	0	NULL	NMDA		stimulation with	increases in					C/EBP		nuclear levels of			NULL		0	NULL	NULL	NULL	gw60_neuron_39_4_625_s_194	12925277	(a1) IGF-1 stimulation maintains low nuclear levels of C/EBP  (lane 2), but levels increase when growth factor support is removed (lane 1) or when L channel or CaMK activities are inhibited (lanes 3 and 4); nimodipine, 5  M; KN62, 10  M. Conversely, NMDA receptor activity increases the levels in a calcineurin-dependent manner: blocking NMDA receptors with 100  M APV reduces nuclear C/EBP  (lane 5), stimulation with 300  M NMDA + 1  M glycine increases it (lane 6), but when 1  M deltamethrin is coapplied, nuclear levels decline (lane 7).	transcription
55629	9	335202	7	NULL	NULL	0	NULL	glycine			increases more than					C/EBP		nuclear levels of			NULL		0	NULL	NULL	NULL	gw60_neuron_39_4_625_s_194	12925277	(a1) IGF-1 stimulation maintains low nuclear levels of C/EBP  (lane 2), but levels increase when growth factor support is removed (lane 1) or when L channel or CaMK activities are inhibited (lanes 3 and 4); nimodipine, 5  M; KN62, 10  M. Conversely, NMDA receptor activity increases the levels in a calcineurin-dependent manner: blocking NMDA receptors with 100  M APV reduces nuclear C/EBP  (lane 5), stimulation with 300  M NMDA + 1  M glycine increases it (lane 6), but when 1  M deltamethrin is coapplied, nuclear levels decline (lane 7).	transcription
55630	10	335202	7	NULL	NULL	0	NULL	statement 8			occur along with					statement 9					NULL		0	NULL	NULL	NULL	gw60_neuron_39_4_625_s_194	12925277	(a1) IGF-1 stimulation maintains low nuclear levels of C/EBP  (lane 2), but levels increase when growth factor support is removed (lane 1) or when L channel or CaMK activities are inhibited (lanes 3 and 4); nimodipine, 5  M; KN62, 10  M. Conversely, NMDA receptor activity increases the levels in a calcineurin-dependent manner: blocking NMDA receptors with 100  M APV reduces nuclear C/EBP  (lane 5), stimulation with 300  M NMDA + 1  M glycine increases it (lane 6), but when 1  M deltamethrin is coapplied, nuclear levels decline (lane 7).	transcription
55631	11	335202	7	NULL	NULL	0	NULL	deltamethrin			decrease					C/EBP		nuclear levels of			NULL		0	NULL	NULL	NULL	gw60_neuron_39_4_625_s_194	12925277	(a1) IGF-1 stimulation maintains low nuclear levels of C/EBP  (lane 2), but levels increase when growth factor support is removed (lane 1) or when L channel or CaMK activities are inhibited (lanes 3 and 4); nimodipine, 5  M; KN62, 10  M. Conversely, NMDA receptor activity increases the levels in a calcineurin-dependent manner: blocking NMDA receptors with 100  M APV reduces nuclear C/EBP  (lane 5), stimulation with 300  M NMDA + 1  M glycine increases it (lane 6), but when 1  M deltamethrin is coapplied, nuclear levels decline (lane 7).	transcription
55632	12	335202	7	NULL	NULL	0	NULL	statement 8			occur along with					statement 11					NULL		0	NULL	NULL	NULL	gw60_neuron_39_4_625_s_194	12925277	(a1) IGF-1 stimulation maintains low nuclear levels of C/EBP  (lane 2), but levels increase when growth factor support is removed (lane 1) or when L channel or CaMK activities are inhibited (lanes 3 and 4); nimodipine, 5  M; KN62, 10  M. Conversely, NMDA receptor activity increases the levels in a calcineurin-dependent manner: blocking NMDA receptors with 100  M APV reduces nuclear C/EBP  (lane 5), stimulation with 300  M NMDA + 1  M glycine increases it (lane 6), but when 1  M deltamethrin is coapplied, nuclear levels decline (lane 7).	transcription
53968	1	335205	5	NULL	NULL	0	NULL	APV			inhibit		selectively			NMDA		responses to			NULL		0	NULL	NULL	NULL	gw60_brainresmolbrainres_93_1_8_s_129	11532333	By comparison, responses to 100  M NMDA plus 10  M glycine, which were inhibited selectively by 100  M APV, were of similar amplitude in oocytes injected with cerebellar mRNA from +/+ and wv/wv mice at P5-6 (+/+ 10 plus-or-minus 5 nA,  n=8 and wv/wv 12 plus-or-minus 5 nA,  n=8), P10 (+/+ 35 plus-or-minus 5 nA,  n=8 and wv/wv 31 plus-or-minus 4 nA,  n=8) or P23 (+/+ 70 plus-or-minus 3 nA,  n=8 and wv/wv 60 plus-or-minus 5 nA,  n=8; second and fourth set of traces in  Fig. 4).	transcription
53969	2	335205	5	NULL	NULL	0	NULL	APV			inhibit		selectively			glycine		responses to			NULL		0	NULL	NULL	NULL	gw60_brainresmolbrainres_93_1_8_s_129	11532333	By comparison, responses to 100  M NMDA plus 10  M glycine, which were inhibited selectively by 100  M APV, were of similar amplitude in oocytes injected with cerebellar mRNA from +/+ and wv/wv mice at P5-6 (+/+ 10 plus-or-minus 5 nA,  n=8 and wv/wv 12 plus-or-minus 5 nA,  n=8), P10 (+/+ 35 plus-or-minus 5 nA,  n=8 and wv/wv 31 plus-or-minus 4 nA,  n=8) or P23 (+/+ 70 plus-or-minus 3 nA,  n=8 and wv/wv 60 plus-or-minus 5 nA,  n=8; second and fourth set of traces in  Fig. 4).	transcription
53970	3	335205	5	NULL	NULL	0	NULL	statement 1			occurs along with					statement 2					NULL		0	NULL	NULL	NULL	gw60_brainresmolbrainres_93_1_8_s_129	11532333	By comparison, responses to 100  M NMDA plus 10  M glycine, which were inhibited selectively by 100  M APV, were of similar amplitude in oocytes injected with cerebellar mRNA from +/+ and wv/wv mice at P5-6 (+/+ 10 plus-or-minus 5 nA,  n=8 and wv/wv 12 plus-or-minus 5 nA,  n=8), P10 (+/+ 35 plus-or-minus 5 nA,  n=8 and wv/wv 31 plus-or-minus 4 nA,  n=8) or P23 (+/+ 70 plus-or-minus 3 nA,  n=8 and wv/wv 60 plus-or-minus 5 nA,  n=8; second and fourth set of traces in  Fig. 4).	transcription
55633	1	335205	7	NULL	NULL	0	NULL	APV			inhibit					NMDA					NULL		0	NULL	NULL	NULL	gw60_brainresmolbrainres_93_1_8_s_129	11532333	By comparison, responses to 100  M NMDA plus 10  M glycine, which were inhibited selectively by 100  M APV, were of similar amplitude in oocytes injected with cerebellar mRNA from +/+ and wv/wv mice at P5-6 (+/+ 10 plus-or-minus 5 nA,  n=8 and wv/wv 12 plus-or-minus 5 nA,  n=8), P10 (+/+ 35 plus-or-minus 5 nA,  n=8 and wv/wv 31 plus-or-minus 4 nA,  n=8) or P23 (+/+ 70 plus-or-minus 3 nA,  n=8 and wv/wv 60 plus-or-minus 5 nA,  n=8; second and fourth set of traces in  Fig. 4).	transcription
55634	2	335205	7	NULL	NULL	0	NULL	APV			inhibit					glycine					NULL		0	NULL	NULL	NULL	gw60_brainresmolbrainres_93_1_8_s_129	11532333	By comparison, responses to 100  M NMDA plus 10  M glycine, which were inhibited selectively by 100  M APV, were of similar amplitude in oocytes injected with cerebellar mRNA from +/+ and wv/wv mice at P5-6 (+/+ 10 plus-or-minus 5 nA,  n=8 and wv/wv 12 plus-or-minus 5 nA,  n=8), P10 (+/+ 35 plus-or-minus 5 nA,  n=8 and wv/wv 31 plus-or-minus 4 nA,  n=8) or P23 (+/+ 70 plus-or-minus 3 nA,  n=8 and wv/wv 60 plus-or-minus 5 nA,  n=8; second and fourth set of traces in  Fig. 4).	transcription
53972	1	335210	5	NULL	NULL	0	NULL	ATP			does not increase					mIPSC		frequency of			NULL	glycinergic presynaptic nerve terminals	NULL	NULL	NULL	NULL	gw60_jneurosci_21_9_2983_s_147	11312282	In the presence of both KT5720 and SP, however, ATP failed to increase the mIPSC frequency (Fig.  5 A,B), indicating that the effect of SP on P2X receptors are not mediated through the PKA pathway in the glycinergic presynaptic nerve terminals.	transcription
53973	2	335210	5	NULL	NULL	0	NULL	statement 1			in the presence of					KT5720 & SP					NULL	glycinergic presynaptic nerve terminals	NULL	NULL	NULL	NULL	gw60_jneurosci_21_9_2983_s_147	11312282	In the presence of both KT5720 and SP, however, ATP failed to increase the mIPSC frequency (Fig.  5 A,B), indicating that the effect of SP on P2X receptors are not mediated through the PKA pathway in the glycinergic presynaptic nerve terminals.	transcription
53976	3	335210	5	NULL	NULL	0	NULL	SP			effects					P2X receptors					NULL	glycinergic presynaptic nerve terminals	NULL	NULL	NULL	NULL	gw60_jneurosci_21_9_2983_s_147	11312282	In the presence of both KT5720 and SP, however, ATP failed to increase the mIPSC frequency (Fig.  5 A,B), indicating that the effect of SP on P2X receptors are not mediated through the PKA pathway in the glycinergic presynaptic nerve terminals.	transcription
53977	4	335210	5	NULL	NULL	0	NULL	statement 3			is not mediated through					PKA pathway					NULL	glycinergic presynaptic nerve terminals	NULL	NULL	NULL	NULL	gw60_jneurosci_21_9_2983_s_147	11312282	In the presence of both KT5720 and SP, however, ATP failed to increase the mIPSC frequency (Fig.  5 A,B), indicating that the effect of SP on P2X receptors are not mediated through the PKA pathway in the glycinergic presynaptic nerve terminals.	transcription
55635	1	335210	7	NULL	NULL	0	NULL	ATP 			does not increase					mIPSC		frequency of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_9_2983_s_147	11312282	In the presence of both KT5720 and SP, however, ATP failed to increase the mIPSC frequency (Fig.  5 A,B), indicating that the effect of SP on P2X receptors are not mediated through the PKA pathway in the glycinergic presynaptic nerve terminals.	transcription
55636	2	335210	7	NULL	NULL	0	NULL	statement 1			in the presence of					KT5720					NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_9_2983_s_147	11312282	In the presence of both KT5720 and SP, however, ATP failed to increase the mIPSC frequency (Fig.  5 A,B), indicating that the effect of SP on P2X receptors are not mediated through the PKA pathway in the glycinergic presynaptic nerve terminals.	transcription
55637	3	335210	7	NULL	NULL	0	NULL	statement 1			in the presence of					SP					NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_9_2983_s_147	11312282	In the presence of both KT5720 and SP, however, ATP failed to increase the mIPSC frequency (Fig.  5 A,B), indicating that the effect of SP on P2X receptors are not mediated through the PKA pathway in the glycinergic presynaptic nerve terminals.	transcription
55638	4	335210	7	NULL	NULL	0	NULL	SP			effect					P2X receptors					NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_9_2983_s_147	11312282	In the presence of both KT5720 and SP, however, ATP failed to increase the mIPSC frequency (Fig.  5 A,B), indicating that the effect of SP on P2X receptors are not mediated through the PKA pathway in the glycinergic presynaptic nerve terminals.	transcription
55639	5	335210	7	NULL	NULL	0	NULL	statement 4			not mediated through					PKA pathway					NULL	glycinergic presynaptic nerve terminals	0	NULL	NULL	NULL	gw60_jneurosci_21_9_2983_s_147	11312282	In the presence of both KT5720 and SP, however, ATP failed to increase the mIPSC frequency (Fig.  5 A,B), indicating that the effect of SP on P2X receptors are not mediated through the PKA pathway in the glycinergic presynaptic nerve terminals.	transcription
53978	1	335213	5	NULL	NULL	0	NULL	3-phosphoglycerate dehydrogenase			is encoded by					serA					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_10_5772_s_155	14532024	Lrp activates 3-phosphoglycerate dehydrogenase (encoded by  serA), which converts the glycolytic intermediate 3-phosphoglycerate to serine, while it represses serine hydroxymethyltransferase (encoded by  glyA) and serine deaminase (encoded by  sdaA) of the serine degradation pathway.	transcription
53979	2	335213	5	NULL	NULL	0	NULL	Lrp			activates					serA					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_10_5772_s_155	14532024	Lrp activates 3-phosphoglycerate dehydrogenase (encoded by  serA), which converts the glycolytic intermediate 3-phosphoglycerate to serine, while it represses serine hydroxymethyltransferase (encoded by  glyA) and serine deaminase (encoded by  sdaA) of the serine degradation pathway.	transcription
53980	3	335213	5	NULL	NULL	0	NULL	3-phosphoglycerate			is a type of					glycolytic intermediate					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_10_5772_s_155	14532024	Lrp activates 3-phosphoglycerate dehydrogenase (encoded by  serA), which converts the glycolytic intermediate 3-phosphoglycerate to serine, while it represses serine hydroxymethyltransferase (encoded by  glyA) and serine deaminase (encoded by  sdaA) of the serine degradation pathway.	transcription
53981	4	335213	5	NULL	NULL	0	NULL	3-phosphoglycerate			is converted to					serine					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_10_5772_s_155	14532024	Lrp activates 3-phosphoglycerate dehydrogenase (encoded by  serA), which converts the glycolytic intermediate 3-phosphoglycerate to serine, while it represses serine hydroxymethyltransferase (encoded by  glyA) and serine deaminase (encoded by  sdaA) of the serine degradation pathway.	transcription
53982	5	335213	5	NULL	NULL	0	NULL	serA			catalyzes					statement 4					NULL		NULL	NULL	NULL	NULL	gw70_applenvironmicrob_69_10_5772_s_155	14532024	Lrp activates 3-phosphoglycerate dehydrogenase (encoded by  serA), which converts the glycolytic intermediate 3-phosphoglycerate to serine, while it represses serine hydroxymethyltransferase (encoded by  glyA) and serine deaminase (encoded by  sdaA) of the serine degradation pathway.	transcription
53983	6	335213	5	NULL	NULL	0	NULL	serine hydroxymethyltransferase			is encoded by					glyA					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_10_5772_s_155	14532024	Lrp activates 3-phosphoglycerate dehydrogenase (encoded by  serA), which converts the glycolytic intermediate 3-phosphoglycerate to serine, while it represses serine hydroxymethyltransferase (encoded by  glyA) and serine deaminase (encoded by  sdaA) of the serine degradation pathway.	transcription
53984	7	335213	5	NULL	NULL	0	NULL	Lrp			repress					glyA					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_10_5772_s_155	14532024	Lrp activates 3-phosphoglycerate dehydrogenase (encoded by  serA), which converts the glycolytic intermediate 3-phosphoglycerate to serine, while it represses serine hydroxymethyltransferase (encoded by  glyA) and serine deaminase (encoded by  sdaA) of the serine degradation pathway.	transcription
53985	8	335213	5	NULL	NULL	0	NULL	Lrp			repress					sdaA					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_10_5772_s_155	14532024	Lrp activates 3-phosphoglycerate dehydrogenase (encoded by  serA), which converts the glycolytic intermediate 3-phosphoglycerate to serine, while it represses serine hydroxymethyltransferase (encoded by  glyA) and serine deaminase (encoded by  sdaA) of the serine degradation pathway.	transcription
53986	9	335213	5	NULL	NULL	0	NULL	serine deaminase			is encoded by					sdaA					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_10_5772_s_155	14532024	Lrp activates 3-phosphoglycerate dehydrogenase (encoded by  serA), which converts the glycolytic intermediate 3-phosphoglycerate to serine, while it represses serine hydroxymethyltransferase (encoded by  glyA) and serine deaminase (encoded by  sdaA) of the serine degradation pathway.	transcription
53987	10	335213	5	NULL	NULL	0	NULL	sdaA			plays a role in					serine degradation pathway					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_10_5772_s_155	14532024	Lrp activates 3-phosphoglycerate dehydrogenase (encoded by  serA), which converts the glycolytic intermediate 3-phosphoglycerate to serine, while it represses serine hydroxymethyltransferase (encoded by  glyA) and serine deaminase (encoded by  sdaA) of the serine degradation pathway.	transcription
53988	11	335213	5	NULL	NULL	0	NULL	glyA			plays a role in					serine degradation pathway					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_10_5772_s_155	14532024	Lrp activates 3-phosphoglycerate dehydrogenase (encoded by  serA), which converts the glycolytic intermediate 3-phosphoglycerate to serine, while it represses serine hydroxymethyltransferase (encoded by  glyA) and serine deaminase (encoded by  sdaA) of the serine degradation pathway.	transcription
55640	1	335213	7	NULL	NULL	0	NULL	Lrp			activates					 3-phosphoglycerate dehydrogenase					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_10_5772_s_155	14532024	Lrp activates 3-phosphoglycerate dehydrogenase (encoded by  serA), which converts the glycolytic intermediate 3-phosphoglycerate to serine, while it represses serine hydroxymethyltransferase (encoded by  glyA) and serine deaminase (encoded by  sdaA) of the serine degradation pathway.	transcription
55641	2	335213	7	NULL	NULL	0	NULL	serA			encodes					 3-phosphoglycerate dehydrogenase					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_10_5772_s_155	14532024	Lrp activates 3-phosphoglycerate dehydrogenase (encoded by  serA), which converts the glycolytic intermediate 3-phosphoglycerate to serine, while it represses serine hydroxymethyltransferase (encoded by  glyA) and serine deaminase (encoded by  sdaA) of the serine degradation pathway.	transcription
55642	3	335213	7	NULL	NULL	0	NULL	glycolytic intermediate 3-phosphoglycerate 			converted to					serine					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_10_5772_s_155	14532024	Lrp activates 3-phosphoglycerate dehydrogenase (encoded by  serA), which converts the glycolytic intermediate 3-phosphoglycerate to serine, while it represses serine hydroxymethyltransferase (encoded by  glyA) and serine deaminase (encoded by  sdaA) of the serine degradation pathway.	transcription
55643	4	335213	7	NULL	NULL	0	NULL	Lrp			repress					serine hydroxymethyltransferase					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_10_5772_s_155	14532024	Lrp activates 3-phosphoglycerate dehydrogenase (encoded by  serA), which converts the glycolytic intermediate 3-phosphoglycerate to serine, while it represses serine hydroxymethyltransferase (encoded by  glyA) and serine deaminase (encoded by  sdaA) of the serine degradation pathway.	transcription
55644	5	335213	7	NULL	NULL	0	NULL	glyA			encode					serine hydroxymethyltransferase					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_10_5772_s_155	14532024	Lrp activates 3-phosphoglycerate dehydrogenase (encoded by  serA), which converts the glycolytic intermediate 3-phosphoglycerate to serine, while it represses serine hydroxymethyltransferase (encoded by  glyA) and serine deaminase (encoded by  sdaA) of the serine degradation pathway.	transcription
55645	6	335213	7	NULL	NULL	0	NULL	3-phosphoglycerate dehydrogenase			catalyse					statement 3					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_10_5772_s_155	14532024	Lrp activates 3-phosphoglycerate dehydrogenase (encoded by  serA), which converts the glycolytic intermediate 3-phosphoglycerate to serine, while it represses serine hydroxymethyltransferase (encoded by  glyA) and serine deaminase (encoded by  sdaA) of the serine degradation pathway.	transcription
55646	7	335213	7	NULL	NULL	0	NULL	Lrp			repress					serine deaminase					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_10_5772_s_155	14532024	Lrp activates 3-phosphoglycerate dehydrogenase (encoded by  serA), which converts the glycolytic intermediate 3-phosphoglycerate to serine, while it represses serine hydroxymethyltransferase (encoded by  glyA) and serine deaminase (encoded by  sdaA) of the serine degradation pathway.	transcription
55647	8	335213	7	NULL	NULL	0	NULL	sdaA			encode					serine deaminase					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_10_5772_s_155	14532024	Lrp activates 3-phosphoglycerate dehydrogenase (encoded by  serA), which converts the glycolytic intermediate 3-phosphoglycerate to serine, while it represses serine hydroxymethyltransferase (encoded by  glyA) and serine deaminase (encoded by  sdaA) of the serine degradation pathway.	transcription
55648	9	335213	7	NULL	NULL	0	NULL	serine hydroxymethyltransferase			belongs to					serine degradation pathway					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_10_5772_s_155	14532024	Lrp activates 3-phosphoglycerate dehydrogenase (encoded by  serA), which converts the glycolytic intermediate 3-phosphoglycerate to serine, while it represses serine hydroxymethyltransferase (encoded by  glyA) and serine deaminase (encoded by  sdaA) of the serine degradation pathway.	transcription
55649	10	335213	7	NULL	NULL	0	NULL	serine deaminase			belongs to					serine degradation pathway					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_10_5772_s_155	14532024	Lrp activates 3-phosphoglycerate dehydrogenase (encoded by  serA), which converts the glycolytic intermediate 3-phosphoglycerate to serine, while it represses serine hydroxymethyltransferase (encoded by  glyA) and serine deaminase (encoded by  sdaA) of the serine degradation pathway.	transcription
53989	1	335214	5	NULL	NULL	0	NULL	PGDH		Escherichia coli	catalyzes					serine biosynthesis		first step of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_eur-j-biochem_269_17_12199695_s_2	12199695	Escherichia coli 3-phosphoglycerate dehydrogenase (PGDH) catalyzes the  first step in serine biosynthesis, and is allosterically inhibited by  serine.	transcription
53990	2	335214	5	NULL	NULL	0	NULL	serine			inhibits		allosterically			PGDH		Escherichia coli			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_eur-j-biochem_269_17_12199695_s_2	12199695	Escherichia coli 3-phosphoglycerate dehydrogenase (PGDH) catalyzes the  first step in serine biosynthesis, and is allosterically inhibited by  serine.	transcription
53991	3	335214	5	NULL	NULL	0	NULL	PGDH			is					3-phosphoglycerate dehydrogenase					NULL		0	NULL	NULL	NULL	abs-batch0650-0679_eur-j-biochem_269_17_12199695_s_2	12199695	Escherichia coli 3-phosphoglycerate dehydrogenase (PGDH) catalyzes the  first step in serine biosynthesis, and is allosterically inhibited by  serine.	transcription
55650	1	335214	7	NULL	NULL	0	NULL	PGDH		Escherichia coli	catalyze					serine		first step in biosynthesis of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_eur-j-biochem_269_17_12199695_s_2	12199695	Escherichia coli 3-phosphoglycerate dehydrogenase (PGDH) catalyzes the  first step in serine biosynthesis, and is allosterically inhibited by  serine.	transcription
55651	2	335214	7	NULL	NULL	0	NULL	serine			inhibits		allosterically			statement 1					NULL		0	NULL	NULL	NULL	abs-batch0650-0679_eur-j-biochem_269_17_12199695_s_2	12199695	Escherichia coli 3-phosphoglycerate dehydrogenase (PGDH) catalyzes the  first step in serine biosynthesis, and is allosterically inhibited by  serine.	transcription
55652	3	335214	7	NULL	NULL	0	NULL	PGDH			is					3-phosphoglycerate dehydrogenase 					NULL		0	NULL	NULL	NULL	abs-batch0650-0679_eur-j-biochem_269_17_12199695_s_2	12199695	Escherichia coli 3-phosphoglycerate dehydrogenase (PGDH) catalyzes the  first step in serine biosynthesis, and is allosterically inhibited by  serine.	transcription
53992	1	335215	5	NULL	NULL	0	NULL	3-phosphoglycerate			is a type of					glycolytic metabolite					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10264_s_3	12525494	These dehydrogenases catalyze the first reaction of serine and glycine biosynthesis from the glycolytic metabolite 3-phosphoglycerate.	transcription
53993	2	335215	5	NULL	NULL	0	NULL	serine			is synthesized from					3-phosphoglycerate					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10264_s_3	12525494	These dehydrogenases catalyze the first reaction of serine and glycine biosynthesis from the glycolytic metabolite 3-phosphoglycerate.	transcription
53994	3	335215	5	NULL	NULL	0	NULL	glycine			is synthesized from					3-phosphoglycerate					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10264_s_3	12525494	These dehydrogenases catalyze the first reaction of serine and glycine biosynthesis from the glycolytic metabolite 3-phosphoglycerate.	transcription
53995	4	335215	5	NULL	NULL	0	NULL	dehydrogenases			catalyzes					statement 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10264_s_3	12525494	These dehydrogenases catalyze the first reaction of serine and glycine biosynthesis from the glycolytic metabolite 3-phosphoglycerate.	transcription
53996	5	335215	5	NULL	NULL	0	NULL	dehydrogenases			catalyzes					statement 3					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10264_s_3	12525494	These dehydrogenases catalyze the first reaction of serine and glycine biosynthesis from the glycolytic metabolite 3-phosphoglycerate.	transcription
55653	1	335215	7	NULL	NULL	0	NULL	 3-phosphoglycerate			is involved in					glycine		biosynthesis of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_12_10264_s_3	12525494	These dehydrogenases catalyze the first reaction of serine and glycine biosynthesis from the glycolytic metabolite 3-phosphoglycerate.	transcription
55654	2	335215	7	NULL	NULL	0	NULL	3-phosphoglycerate			is a type of					glycolytic metabolite					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_12_10264_s_3	12525494	These dehydrogenases catalyze the first reaction of serine and glycine biosynthesis from the glycolytic metabolite 3-phosphoglycerate.	transcription
53997	1	335216	5	NULL	NULL	0	NULL	threonine deaminase		structure of	resembles			C-domain		3-phosphoglycerate dehydrogenase			serine binding domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_18_12855_s_256	10212273	The structure of the C-domain of threonine deaminase resembles that of the serine binding domain of 3-phosphoglycerate dehydrogenase.	transcription
56146	1	335216	7	NULL	NULL	0	NULL	threonine deaminase			resembles			C-domain 		3-phosphoglycerate dehydrogenase			serine binding domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_18_12855_s_256	10212273	The structure of the C-domain of threonine deaminase resembles that of the serine binding domain of 3-phosphoglycerate dehydrogenase.	transcription
53998	1	335217	5	NULL	NULL	0	NULL	3-phosphoglycerate			is oxidized to					phosphohydroxypyruvate					NULL		0	NULL	NULL	NULL	gw70_pnas_100_1_370_s_175	12509500	An enzyme of nitrogen metabolism has been identified as a potential target for thioredoxin:  phosphoglycerate dehydrogenase, which catalyzes the oxidation of 3-phosphoglycerate to phosphohydroxypyruvate in the first step of the serine biosynthesis.	transcription
53999	2	335217	5	NULL	NULL	0	NULL	statement 1			is first step of					serine		biosynthesis of			NULL		0	NULL	NULL	NULL	gw70_pnas_100_1_370_s_175	12509500	An enzyme of nitrogen metabolism has been identified as a potential target for thioredoxin:  phosphoglycerate dehydrogenase, which catalyzes the oxidation of 3-phosphoglycerate to phosphohydroxypyruvate in the first step of the serine biosynthesis.	transcription
54000	3	335217	5	NULL	NULL	0	NULL	phosphoglycerate dehydrogenase			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw70_pnas_100_1_370_s_175	12509500	An enzyme of nitrogen metabolism has been identified as a potential target for thioredoxin:  phosphoglycerate dehydrogenase, which catalyzes the oxidation of 3-phosphoglycerate to phosphohydroxypyruvate in the first step of the serine biosynthesis.	transcription
54001	4	335217	5	NULL	NULL	0	NULL	phosphoglycerate dehydrogenase			target for		potential			thioredoxin					NULL		0	NULL	NULL	NULL	gw70_pnas_100_1_370_s_175	12509500	An enzyme of nitrogen metabolism has been identified as a potential target for thioredoxin:  phosphoglycerate dehydrogenase, which catalyzes the oxidation of 3-phosphoglycerate to phosphohydroxypyruvate in the first step of the serine biosynthesis.	transcription
55655	1	335217	7	NULL	NULL	0	NULL	3-phosphoglycerate			oxidizes to					phosphohydroxypyruvate					NULL		0	NULL	NULL	NULL	gw70_pnas_100_1_370_s_175	12509500	An enzyme of nitrogen metabolism has been identified as a potential target for thioredoxin:  phosphoglycerate dehydrogenase, which catalyzes the oxidation of 3-phosphoglycerate to phosphohydroxypyruvate in the first step of the serine biosynthesis.	transcription
55656	2	335217	7	NULL	NULL	0	NULL	statement 1			first step in the					serine		biosynthesis of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_1_370_s_175	12509500	An enzyme of nitrogen metabolism has been identified as a potential target for thioredoxin:  phosphoglycerate dehydrogenase, which catalyzes the oxidation of 3-phosphoglycerate to phosphohydroxypyruvate in the first step of the serine biosynthesis.	transcription
55657	3	335217	7	NULL	NULL	0	NULL	nitrogen metabolism enzyme			potential target for					thioredoxin					NULL		0	NULL	NULL	NULL	gw70_pnas_100_1_370_s_175	12509500	An enzyme of nitrogen metabolism has been identified as a potential target for thioredoxin:  phosphoglycerate dehydrogenase, which catalyzes the oxidation of 3-phosphoglycerate to phosphohydroxypyruvate in the first step of the serine biosynthesis.	transcription
54002	1	335218	5	NULL	NULL	0	NULL	Upp			is					uracil phosphoribosyltransferase					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_39_29131_s_217	16893888	Uracil phosphoribosyltransferase (Upp) functions to regulate entry into the pyrimidine salvage pathway commonly induced by starvation conditions, whereas SerA (D-3-phosphoglycerate dehydrogenase) regulates the cellular levels of 3-phosphoglycerate from serine.	transcription
54003	2	335218	5	NULL	NULL	0	NULL	Upp			regulates					pyrimidine salvage pathway		entry into			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_39_29131_s_217	16893888	Uracil phosphoribosyltransferase (Upp) functions to regulate entry into the pyrimidine salvage pathway commonly induced by starvation conditions, whereas SerA (D-3-phosphoglycerate dehydrogenase) regulates the cellular levels of 3-phosphoglycerate from serine.	transcription
54004	3	335218	5	NULL	NULL	0	NULL	pyrimidine salvage pathway			is induced by		commonly			starvation					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_39_29131_s_217	16893888	Uracil phosphoribosyltransferase (Upp) functions to regulate entry into the pyrimidine salvage pathway commonly induced by starvation conditions, whereas SerA (D-3-phosphoglycerate dehydrogenase) regulates the cellular levels of 3-phosphoglycerate from serine.	transcription
54005	4	335218	5	NULL	NULL	0	NULL	SerA			is					D-3-phosphoglycerate dehydrogenase					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_39_29131_s_217	16893888	Uracil phosphoribosyltransferase (Upp) functions to regulate entry into the pyrimidine salvage pathway commonly induced by starvation conditions, whereas SerA (D-3-phosphoglycerate dehydrogenase) regulates the cellular levels of 3-phosphoglycerate from serine.	transcription
54006	5	335218	5	NULL	NULL	0	NULL	3-phosphoglycerate			is obtained from					serine					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_39_29131_s_217	16893888	Uracil phosphoribosyltransferase (Upp) functions to regulate entry into the pyrimidine salvage pathway commonly induced by starvation conditions, whereas SerA (D-3-phosphoglycerate dehydrogenase) regulates the cellular levels of 3-phosphoglycerate from serine.	transcription
54007	6	335218	5	NULL	NULL	0	NULL	SerA			regulates					statement 5		cellular levels of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_39_29131_s_217	16893888	Uracil phosphoribosyltransferase (Upp) functions to regulate entry into the pyrimidine salvage pathway commonly induced by starvation conditions, whereas SerA (D-3-phosphoglycerate dehydrogenase) regulates the cellular levels of 3-phosphoglycerate from serine.	transcription
55658	1	335218	7	NULL	NULL	0	NULL	D-3-phosphoglycerate			is obtained from					serine					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_39_29131_s_217	16893888	Uracil phosphoribosyltransferase (Upp) functions to regulate entry into the pyrimidine salvage pathway commonly induced by starvation conditions, whereas SerA (D-3-phosphoglycerate dehydrogenase) regulates the cellular levels of 3-phosphoglycerate from serine.	transcription
55659	2	335218	7	NULL	NULL	0	NULL	SerA			regulates					statement 1		cellular levels of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_39_29131_s_217	16893888	Uracil phosphoribosyltransferase (Upp) functions to regulate entry into the pyrimidine salvage pathway commonly induced by starvation conditions, whereas SerA (D-3-phosphoglycerate dehydrogenase) regulates the cellular levels of 3-phosphoglycerate from serine.	transcription
55660	3	335218	7	NULL	NULL	0	NULL	Upp			regulate					pyrimidine salvage pathway		entry into			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_39_29131_s_217	16893888	Uracil phosphoribosyltransferase (Upp) functions to regulate entry into the pyrimidine salvage pathway commonly induced by starvation conditions, whereas SerA (D-3-phosphoglycerate dehydrogenase) regulates the cellular levels of 3-phosphoglycerate from serine.	transcription
55661	4	335218	7	NULL	NULL	0	NULL	statement 3			induced by					starvation condition					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_39_29131_s_217	16893888	Uracil phosphoribosyltransferase (Upp) functions to regulate entry into the pyrimidine salvage pathway commonly induced by starvation conditions, whereas SerA (D-3-phosphoglycerate dehydrogenase) regulates the cellular levels of 3-phosphoglycerate from serine.	transcription
55662	5	335218	7	NULL	NULL	0	NULL	UPP			is					Uracil phosphoribosyltransferase					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_39_29131_s_217	16893888	Uracil phosphoribosyltransferase (Upp) functions to regulate entry into the pyrimidine salvage pathway commonly induced by starvation conditions, whereas SerA (D-3-phosphoglycerate dehydrogenase) regulates the cellular levels of 3-phosphoglycerate from serine.	transcription
55663	6	335218	7	NULL	NULL	0	NULL	SerA			is					D-3-phosphoglycerate dehydrogenase					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_39_29131_s_217	16893888	Uracil phosphoribosyltransferase (Upp) functions to regulate entry into the pyrimidine salvage pathway commonly induced by starvation conditions, whereas SerA (D-3-phosphoglycerate dehydrogenase) regulates the cellular levels of 3-phosphoglycerate from serine.	transcription
54008	1	335219	5	NULL	NULL	0	NULL	p105			processed to					p50					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_4_980_s_107	13679070	Casper inhibits the processing of p105 to p50	transcription
54009	2	335219	5	NULL	NULL	0	NULL	Casper			inhibits					statement 1					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_4_980_s_107	13679070	Casper inhibits the processing of p105 to p50	transcription
55664	1	335219	7	NULL	NULL	0	NULL	p105			processed to					p50					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_4_980_s_107	13679070	Casper inhibits the processing of p105 to p50	transcription
55665	2	335219	7	NULL	NULL	0	NULL	Casper			inhibits					statement 1					NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_4_980_s_107	13679070	Casper inhibits the processing of p105 to p50	transcription
54010	1	335220	5	NULL	NULL	0	NULL	p105.p50 complex			is retained in					cytoplasm					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_1_556_s_421	12399470	Expression of p105 or both p105 and p50 results in a p105.p50 complex that is retained in the cytoplasm.	transcription
54011	2	335220	5	NULL	NULL	0	NULL	p105 & p50		expression of	results in					p105.p50 complex					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_1_556_s_421	12399470	Expression of p105 or both p105 and p50 results in a p105.p50 complex that is retained in the cytoplasm.	transcription
55666	1	335220	7	NULL	NULL	0	NULL	p105		expression of	results in					p105.p50 complex					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_1_556_s_421	12399470	Expression of p105 or both p105 and p50 results in a p105.p50 complex that is retained in the cytoplasm.	transcription
55667	2	335220	7	NULL	NULL	0	NULL	p50		expression of	results in					p105.p50 complex					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_1_556_s_421	12399470	Expression of p105 or both p105 and p50 results in a p105.p50 complex that is retained in the cytoplasm.	transcription
55668	3	335220	7	NULL	NULL	0	NULL	statement 1			occur along with					statement 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_1_556_s_421	12399470	Expression of p105 or both p105 and p50 results in a p105.p50 complex that is retained in the cytoplasm.	transcription
55669	4	335220	7	NULL	NULL	0	NULL	statement 3			results in					p105.p50 complex					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_1_556_s_421	12399470	Expression of p105 or both p105 and p50 results in a p105.p50 complex that is retained in the cytoplasm.	transcription
55670	5	335220	7	NULL	NULL	0	NULL	statement 4			is an alternative to					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_1_556_s_421	12399470	Expression of p105 or both p105 and p50 results in a p105.p50 complex that is retained in the cytoplasm.	transcription
55671	6	335220	7	NULL	NULL	0	NULL	p105.p50 complex			retained in					cytoplasm					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_1_556_s_421	12399470	Expression of p105 or both p105 and p50 results in a p105.p50 complex that is retained in the cytoplasm.	transcription
54013	1	335221	5	NULL	NULL	0	NULL	proteolysis			leads to					p50		generation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_126	12807880	Proteolysis Leading to p50 Generation Initiates at an Internal Site of  the p105 Protein --	transcription
55672	1	335221	7	NULL	NULL	0	NULL	proteolysis			leads to					p50		generation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_126	12807880	Proteolysis Leading to p50 Generation Initiates at an Internal Site of  the p105 Protein --	transcription
55673	2	335221	7	NULL	NULL	0	NULL	statement 1			initiates					p105 Protein			Internal Site of		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_126	12807880	Proteolysis Leading to p50 Generation Initiates at an Internal Site of  the p105 Protein --	transcription
54014	1	335222	5	NULL	NULL	0	NULL	IKK			stimulates					p105		processing of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_222	11350967	Panel A, IKK stimulates processing of p105 and subsequent translocation of the resulting p50 to the nucleus.	transcription
54015	2	335222	5	NULL	NULL	0	NULL	p50			is translocated to					nucleus					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_222	11350967	Panel A, IKK stimulates processing of p105 and subsequent translocation of the resulting p50 to the nucleus.	transcription
54016	3	335222	5	NULL	NULL	0	NULL	IKK			stimulates		subsequently			statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_222	11350967	Panel A, IKK stimulates processing of p105 and subsequent translocation of the resulting p50 to the nucleus.	transcription
55674	1	335222	7	NULL	NULL	0	NULL	 IKK 			stimulates					p105		processing of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_222	11350967	Panel A, IKK stimulates processing of p105 and subsequent translocation of the resulting p50 to the nucleus.	transcription
55675	2	335222	7	NULL	NULL	0	NULL	p50			translocated to					nucleus					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_222	11350967	Panel A, IKK stimulates processing of p105 and subsequent translocation of the resulting p50 to the nucleus.	transcription
55676	3	335222	7	NULL	NULL	0	NULL	statement 1			leads to					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_222	11350967	Panel A, IKK stimulates processing of p105 and subsequent translocation of the resulting p50 to the nucleus.	transcription
54566	1	335223	5	NULL	NULL	0	NULL	Casper			interacts with					p105					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_4_980_s_108	13679070	Since Casper interacts with p105, we examined whether Casper has any effects on p105  processing into p50.	transcription
54567	2	335223	5	NULL	NULL	0	NULL	p105			is processed into					p50					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_4_980_s_108	13679070	Since Casper interacts with p105, we examined whether Casper has any effects on p105  processing into p50.	transcription
54568	3	335223	5	NULL	NULL	0	NULL	Casper			effect		may			statement 2					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_4_980_s_108	13679070	Since Casper interacts with p105, we examined whether Casper has any effects on p105  processing into p50.	transcription
55677	1	335223	7	NULL	NULL	0	NULL	Casper			interacts with					p105					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_4_980_s_108	13679070	Since Casper interacts with p105, we examined whether Casper has any effects on p105  processing into p50.	transcription
54569	1	335224	5	NULL	NULL	0	NULL	Tpl-2			interacts with		directly			p105					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_32465_s_206	12801933	Tpl-2 directly  interacts with p105, and its overexpression leads to increased turnover of  p105 into p50 subunits ( ).	transcription
54570	2	335224	5	NULL	NULL	0	NULL	p105			is converted to					p50 subunits					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_32465_s_206	12801933	Tpl-2 directly  interacts with p105, and its overexpression leads to increased turnover of  p105 into p50 subunits ( ).	transcription
54571	3	335224	5	NULL	NULL	0	NULL	Tpl-2		overexpression of	leads to					statement 2		increased			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_34_32465_s_206	12801933	Tpl-2 directly  interacts with p105, and its overexpression leads to increased turnover of  p105 into p50 subunits ( ).	transcription
55678	1	335224	7	NULL	NULL	0	NULL	Tpl-2			interacts with		directly			p105					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_32465_s_206	12801933	Tpl-2 directly  interacts with p105, and its overexpression leads to increased turnover of  p105 into p50 subunits ( ).	transcription
55679	2	335224	7	NULL	NULL	0	NULL	p105			converted to					p50 subunits					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_32465_s_206	12801933	Tpl-2 directly  interacts with p105, and its overexpression leads to increased turnover of  p105 into p50 subunits ( ).	transcription
55680	3	335224	7	NULL	NULL	0	NULL	Tpl-2		overexpression of	increase					statement 2		turnover of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_34_32465_s_206	12801933	Tpl-2 directly  interacts with p105, and its overexpression leads to increased turnover of  p105 into p50 subunits ( ).	transcription
54572	1	335226	5	NULL	NULL	0	NULL	p50			inhibits					p105		processing of	ankyrin repeat		NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_189	11350967	p50 inhibits  in vivo processing of ankyrin repeat-containing, but not of ankyrin repeat-lacking p105s.	transcription
54573	2	335226	5	NULL	NULL	0	NULL	p105			lacks								ankyrin repeat		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_189	11350967	p50 inhibits  in vivo processing of ankyrin repeat-containing, but not of ankyrin repeat-lacking p105s.	transcription
54574	3	335226	5	NULL	NULL	0	NULL	p50			does not inhibit					statement 2		processing of			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_189	11350967	p50 inhibits  in vivo processing of ankyrin repeat-containing, but not of ankyrin repeat-lacking p105s.	transcription
55681	1	335226	7	NULL	NULL	0	NULL	 p105			contains					ankyrin repeat					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_189	11350967	p50 inhibits  in vivo processing of ankyrin repeat-containing, but not of ankyrin repeat-lacking p105s.	transcription
55682	2	335226	7	NULL	NULL	0	NULL	p50			inhibits					statement 1		in vivo processing of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_189	11350967	p50 inhibits  in vivo processing of ankyrin repeat-containing, but not of ankyrin repeat-lacking p105s.	transcription
55683	3	335226	7	NULL	NULL	0	NULL	p105			lacks								ankyrin repeat		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_189	11350967	p50 inhibits  in vivo processing of ankyrin repeat-containing, but not of ankyrin repeat-lacking p105s.	transcription
55684	4	335226	7	NULL	NULL	0	NULL	p50			does not inhibit					statement 3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_189	11350967	p50 inhibits  in vivo processing of ankyrin repeat-containing, but not of ankyrin repeat-lacking p105s.	transcription
54575	1	335227	5	NULL	NULL	0	NULL	p105			is processed into					p50					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_52_54841_s_33	15485831	Processing of p105 into p50 is constitutively regulated, and p50 is most commonly associated with p65 and the inhibitor protein IkappaBalpha in an inactive complex in the cytosol.	transcription
54576	2	335227	5	NULL	NULL	0	NULL	p50			is associated with		most commonly			p65					NULL	cytosol	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_52_54841_s_33	15485831	Processing of p105 into p50 is constitutively regulated, and p50 is most commonly associated with p65 and the inhibitor protein IkappaBalpha in an inactive complex in the cytosol.	transcription
54577	3	335227	5	NULL	NULL	0	NULL	p50			is associated with		most commonly			IkappaBalpha					NULL	cytosol	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_52_54841_s_33	15485831	Processing of p105 into p50 is constitutively regulated, and p50 is most commonly associated with p65 and the inhibitor protein IkappaBalpha in an inactive complex in the cytosol.	transcription
54578	4	335227	5	NULL	NULL	0	NULL	statement 2			occurs along with					statement 3					NULL	cytosol	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_52_54841_s_33	15485831	Processing of p105 into p50 is constitutively regulated, and p50 is most commonly associated with p65 and the inhibitor protein IkappaBalpha in an inactive complex in the cytosol.	transcription
54579	5	335227	5	NULL	NULL	0	NULL	statement 4			forms					complex		inactive			NULL	cytosol	0	NULL	NULL	NULL	gw70_jbiolchem_279_52_54841_s_33	15485831	Processing of p105 into p50 is constitutively regulated, and p50 is most commonly associated with p65 and the inhibitor protein IkappaBalpha in an inactive complex in the cytosol.	transcription
54580	6	335227	5	NULL	NULL	0	NULL	IkappaBalpha			is a type of					inhibitor protein					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_52_54841_s_33	15485831	Processing of p105 into p50 is constitutively regulated, and p50 is most commonly associated with p65 and the inhibitor protein IkappaBalpha in an inactive complex in the cytosol.	transcription
55685	1	335227	7	NULL	NULL	0	NULL	p105			processed to					p50					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_52_54841_s_33	15485831	Processing of p105 into p50 is constitutively regulated, and p50 is most commonly associated with p65 and the inhibitor protein IkappaBalpha in an inactive complex in the cytosol.	transcription
55686	2	335227	7	NULL	NULL	0	NULL	p50			associate with					p65					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_52_54841_s_33	15485831	Processing of p105 into p50 is constitutively regulated, and p50 is most commonly associated with p65 and the inhibitor protein IkappaBalpha in an inactive complex in the cytosol.	transcription
55687	3	335227	7	NULL	NULL	0	NULL	p50			associate with					IkappaBalpha					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_52_54841_s_33	15485831	Processing of p105 into p50 is constitutively regulated, and p50 is most commonly associated with p65 and the inhibitor protein IkappaBalpha in an inactive complex in the cytosol.	transcription
55688	4	335227	7	NULL	NULL	0	NULL	statement 2			occur in an					inactive complex					NULL	cytosol	0	NULL	NULL	NULL	gw70_jbiolchem_279_52_54841_s_33	15485831	Processing of p105 into p50 is constitutively regulated, and p50 is most commonly associated with p65 and the inhibitor protein IkappaBalpha in an inactive complex in the cytosol.	transcription
55689	5	335227	7	NULL	NULL	0	NULL	statement 3			occur in an					inactive complex					NULL	cytosol	0	NULL	NULL	NULL	gw70_jbiolchem_279_52_54841_s_33	15485831	Processing of p105 into p50 is constitutively regulated, and p50 is most commonly associated with p65 and the inhibitor protein IkappaBalpha in an inactive complex in the cytosol.	transcription
55690	6	335227	7	NULL	NULL	0	NULL	statement 1		processing of	regulated					constitutively					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_52_54841_s_33	15485831	Processing of p105 into p50 is constitutively regulated, and p50 is most commonly associated with p65 and the inhibitor protein IkappaBalpha in an inactive complex in the cytosol.	transcription
55691	7	335227	7	NULL	NULL	0	NULL	IkappaBalpha			is a type of					inhibitor protein					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_52_54841_s_33	15485831	Processing of p105 into p50 is constitutively regulated, and p50 is most commonly associated with p65 and the inhibitor protein IkappaBalpha in an inactive complex in the cytosol.	transcription
54581	1	335228	5	NULL	NULL	0	NULL	p50			is generated by		cotranslationally			proteasome-mediated process					NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_27	9529257	Rather, p50 is generated cotranslationally by a proteasome-mediated process that ensures the  production of both p50 and p105 and preserves their independent functions.	transcription
54582	2	335228	5	NULL	NULL	0	NULL	statement 1			ensures					p50		production of			NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_27	9529257	Rather, p50 is generated cotranslationally by a proteasome-mediated process that ensures the  production of both p50 and p105 and preserves their independent functions.	transcription
54583	3	335228	5	NULL	NULL	0	NULL	statement 1			ensures					p105		production of			NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_27	9529257	Rather, p50 is generated cotranslationally by a proteasome-mediated process that ensures the  production of both p50 and p105 and preserves their independent functions.	transcription
54584	4	335228	5	NULL	NULL	0	NULL	statement 2			occurs along with					statement 3					NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_27	9529257	Rather, p50 is generated cotranslationally by a proteasome-mediated process that ensures the  production of both p50 and p105 and preserves their independent functions.	transcription
55692	1	335228	7	NULL	NULL	0	NULL	proteasome-mediated process 			generates		cotranslationally			p50					NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_27	9529257	Rather, p50 is generated cotranslationally by a proteasome-mediated process that ensures the  production of both p50 and p105 and preserves their independent functions.	transcription
55693	2	335228	7	NULL	NULL	0	NULL	statement 1			ensures					p50		production of			NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_27	9529257	Rather, p50 is generated cotranslationally by a proteasome-mediated process that ensures the  production of both p50 and p105 and preserves their independent functions.	transcription
55694	3	335228	7	NULL	NULL	0	NULL	statement 1			ensures					p105		production of			NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_27	9529257	Rather, p50 is generated cotranslationally by a proteasome-mediated process that ensures the  production of both p50 and p105 and preserves their independent functions.	transcription
55695	4	335228	7	NULL	NULL	0	NULL	statement 1			preserves					p50		independent function of			NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_27	9529257	Rather, p50 is generated cotranslationally by a proteasome-mediated process that ensures the  production of both p50 and p105 and preserves their independent functions.	transcription
55696	5	335228	7	NULL	NULL	0	NULL	statement 1			preserves					p105		independent function of			NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_27	9529257	Rather, p50 is generated cotranslationally by a proteasome-mediated process that ensures the  production of both p50 and p105 and preserves their independent functions.	transcription
54585	1	335229	5	NULL	NULL	0	NULL	p105			is a type of					NF- B p50 precursor					NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_472	9529257	The NF- B p50 precursor, p105, contains an internal I B-like inhibitor that preferentially inhibits p50.	transcription
54586	2	335229	5	NULL	NULL	0	NULL	p105			contains					I B-like inhibitor		internal			NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_472	9529257	The NF- B p50 precursor, p105, contains an internal I B-like inhibitor that preferentially inhibits p50.	transcription
54587	3	335229	5	NULL	NULL	0	NULL	statement 2			inhibits		preferentially			p50					NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_472	9529257	The NF- B p50 precursor, p105, contains an internal I B-like inhibitor that preferentially inhibits p50.	transcription
55697	1	335229	7	NULL	NULL	0	NULL	NF- B p50			precursor of					p105					NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_472	9529257	The NF- B p50 precursor, p105, contains an internal I B-like inhibitor that preferentially inhibits p50.	transcription
55698	2	335229	7	NULL	NULL	0	NULL	p105			contains					internal I B-like inhibitor					NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_472	9529257	The NF- B p50 precursor, p105, contains an internal I B-like inhibitor that preferentially inhibits p50.	transcription
55699	3	335229	7	NULL	NULL	0	NULL	p105			inhibits		preferentially			p50					NULL		NULL	NULL	NULL	NULL	gw60_cell_92_6_819_s_472	9529257	The NF- B p50 precursor, p105, contains an internal I B-like inhibitor that preferentially inhibits p50.	transcription
54588	1	335230	5	NULL	NULL	0	NULL	p50			is translocated to					nucleus					NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_69	9950430	Thus, TPL2-mediated activation of nuclear translocation of p50 does not require stimulation of p105 processing to p50.	transcription
54589	2	335230	5	NULL	NULL	0	NULL	TPL2			mediates					statement 1		activation of			NULL		NULL	NULL	NULL	NULL	gw60_nature_397_6717_363_s_69	9950430	Thus, TPL2-mediated activation of nuclear translocation of p50 does not require stimulation of p105 processing to p50.	transcription
54590	3	335230	5	NULL	NULL	0	NULL	p105			is processed to					p50					NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_69	9950430	Thus, TPL2-mediated activation of nuclear translocation of p50 does not require stimulation of p105 processing to p50.	transcription
54591	4	335230	5	NULL	NULL	0	NULL	statement 2			does not require					statement 3		stimulation of			NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_69	9950430	Thus, TPL2-mediated activation of nuclear translocation of p50 does not require stimulation of p105 processing to p50.	transcription
55700	1	335230	7	NULL	NULL	0	NULL	p105			processed to					p50					NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_69	9950430	Thus, TPL2-mediated activation of nuclear translocation of p50 does not require stimulation of p105 processing to p50.	transcription
55701	2	335230	7	NULL	NULL	0	NULL	TPL2			mediates					p50		activation of ;; nuclear translocation of			NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_69	9950430	Thus, TPL2-mediated activation of nuclear translocation of p50 does not require stimulation of p105 processing to p50.	transcription
55702	3	335230	7	NULL	NULL	0	NULL	statement 2			does not require					statement 1		stimulation of			NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_69	9950430	Thus, TPL2-mediated activation of nuclear translocation of p50 does not require stimulation of p105 processing to p50.	transcription
54601	1	335231	5	NULL	NULL	0	NULL	p105			undergoes					processing					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_190	11350967	Panel A, processing of p105 and nuclear translocation of p50 are inhibited by the presence of an ankyrin repeat domain that binds p50.	transcription
54602	2	335231	5	NULL	NULL	0	NULL	p50			is translocated to					nucleus					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_190	11350967	Panel A, processing of p105 and nuclear translocation of p50 are inhibited by the presence of an ankyrin repeat domain that binds p50.	transcription
54603	3	335231	5	NULL	NULL	0	NULL				bind			ankyrin repeat domain		p50					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_190	11350967	Panel A, processing of p105 and nuclear translocation of p50 are inhibited by the presence of an ankyrin repeat domain that binds p50.	transcription
54604	4	335231	5	NULL	NULL	0	NULL	statement 3		presence of	inhibits					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_190	11350967	Panel A, processing of p105 and nuclear translocation of p50 are inhibited by the presence of an ankyrin repeat domain that binds p50.	transcription
54605	5	335231	5	NULL	NULL	0	NULL	statement 3		presence of	inhibits					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_190	11350967	Panel A, processing of p105 and nuclear translocation of p50 are inhibited by the presence of an ankyrin repeat domain that binds p50.	transcription
55703	1	335231	7	NULL	NULL	0	NULL				bind			 ankyrin repeat domain		p50					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_190	11350967	Panel A, processing of p105 and nuclear translocation of p50 are inhibited by the presence of an ankyrin repeat domain that binds p50.	transcription
55704	2	335231	7	NULL	NULL	0	NULL			presence of	inhibits			ankyrin repeat domain		p105		processing of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_190	11350967	Panel A, processing of p105 and nuclear translocation of p50 are inhibited by the presence of an ankyrin repeat domain that binds p50.	transcription
55705	3	335231	7	NULL	NULL	0	NULL			presence of	inhibits			ankyrin repeat domain		p50		nuclear translocation of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_190	11350967	Panel A, processing of p105 and nuclear translocation of p50 are inhibited by the presence of an ankyrin repeat domain that binds p50.	transcription
54606	1	335232	5	NULL	NULL	0	NULL	Bcl-3			bind					p50 dimers					NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_270	10469655	Bcl-3-bound p50 dimers are in fact a suitable readout system for p105-controlled Rel activity: in contrast to Bcl-3, neither IkappaBalpha, beta nor   binds to p50 efficiently and p50 is produced from processed p105 and sequestered by p105.	transcription
54607	2	335232	5	NULL	NULL	0	NULL	Rel		activity of	is controlled by					p105					NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_270	10469655	Bcl-3-bound p50 dimers are in fact a suitable readout system for p105-controlled Rel activity: in contrast to Bcl-3, neither IkappaBalpha, beta nor   binds to p50 efficiently and p50 is produced from processed p105 and sequestered by p105.	transcription
54608	3	335232	5	NULL	NULL	0	NULL	IkappaBalpha			does not bind		efficiently			p50					NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_270	10469655	Bcl-3-bound p50 dimers are in fact a suitable readout system for p105-controlled Rel activity: in contrast to Bcl-3, neither IkappaBalpha, beta nor   binds to p50 efficiently and p50 is produced from processed p105 and sequestered by p105.	transcription
54609	4	335232	5	NULL	NULL	0	NULL	IkappaBbeta			does not bind		efficiently			p50					NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_270	10469655	Bcl-3-bound p50 dimers are in fact a suitable readout system for p105-controlled Rel activity: in contrast to Bcl-3, neither IkappaBalpha, beta nor   binds to p50 efficiently and p50 is produced from processed p105 and sequestered by p105.	transcription
54610	5	335232	5	NULL	NULL	0	NULL	p50			is produced from					p105		processed			NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_270	10469655	Bcl-3-bound p50 dimers are in fact a suitable readout system for p105-controlled Rel activity: in contrast to Bcl-3, neither IkappaBalpha, beta nor   binds to p50 efficiently and p50 is produced from processed p105 and sequestered by p105.	transcription
54611	6	335232	5	NULL	NULL	0	NULL	p50			is sequestered by					p105					NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_270	10469655	Bcl-3-bound p50 dimers are in fact a suitable readout system for p105-controlled Rel activity: in contrast to Bcl-3, neither IkappaBalpha, beta nor   binds to p50 efficiently and p50 is produced from processed p105 and sequestered by p105.	transcription
55706	1	335232	7	NULL	NULL	0	NULL	Bcl-3-			bind					p50 dimers					NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_270	10469655	Bcl-3-bound p50 dimers are in fact a suitable readout system for p105-controlled Rel activity: in contrast to Bcl-3, neither IkappaBalpha, beta nor   binds to p50 efficiently and p50 is produced from processed p105 and sequestered by p105.	transcription
55707	2	335232	7	NULL	NULL	0	NULL	IkappaBalpha			does not bind		efficiently			p50					NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_270	10469655	Bcl-3-bound p50 dimers are in fact a suitable readout system for p105-controlled Rel activity: in contrast to Bcl-3, neither IkappaBalpha, beta nor   binds to p50 efficiently and p50 is produced from processed p105 and sequestered by p105.	transcription
55708	3	335232	7	NULL	NULL	0	NULL	IkappaBbeta			does not bind		efficiently			p50					NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_270	10469655	Bcl-3-bound p50 dimers are in fact a suitable readout system for p105-controlled Rel activity: in contrast to Bcl-3, neither IkappaBalpha, beta nor   binds to p50 efficiently and p50 is produced from processed p105 and sequestered by p105.	transcription
55709	4	335232	7	NULL	NULL	0	NULL	p105			controls					Rel		activity of			NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_270	10469655	Bcl-3-bound p50 dimers are in fact a suitable readout system for p105-controlled Rel activity: in contrast to Bcl-3, neither IkappaBalpha, beta nor   binds to p50 efficiently and p50 is produced from processed p105 and sequestered by p105.	transcription
55710	5	335232	7	NULL	NULL	0	NULL	p50			produced from					p105		processed			NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_270	10469655	Bcl-3-bound p50 dimers are in fact a suitable readout system for p105-controlled Rel activity: in contrast to Bcl-3, neither IkappaBalpha, beta nor   binds to p50 efficiently and p50 is produced from processed p105 and sequestered by p105.	transcription
55711	6	335232	7	NULL	NULL	0	NULL	p50			sequestered by					p105					NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_270	10469655	Bcl-3-bound p50 dimers are in fact a suitable readout system for p105-controlled Rel activity: in contrast to Bcl-3, neither IkappaBalpha, beta nor   binds to p50 efficiently and p50 is produced from processed p105 and sequestered by p105.	transcription
54612	1	335233	5	NULL	NULL	0	NULL	p105 protein			undergoes					proteolysis					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_135	12807880	To demonstrate that proteolysis leading to p50 generation initiates at the  internal site of the p105 protein, we expressed the N-terminal 530 residues of  p105 in the cell.	transcription
54613	2	335233	5	NULL	NULL	0	NULL	statement 1			generates					p50					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_135	12807880	To demonstrate that proteolysis leading to p50 generation initiates at the  internal site of the p105 protein, we expressed the N-terminal 530 residues of  p105 in the cell.	transcription
55713	1	335233	7	NULL	NULL	0	NULL	proteloysis			generates					p50					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_135	12807880	To demonstrate that proteolysis leading to p50 generation initiates at the  internal site of the p105 protein, we expressed the N-terminal 530 residues of  p105 in the cell.	transcription
55714	2	335233	7	NULL	NULL	0	NULL	statement 1			initiates					p105 protein		internal site of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_135	12807880	To demonstrate that proteolysis leading to p50 generation initiates at the  internal site of the p105 protein, we expressed the N-terminal 530 residues of  p105 in the cell.	transcription
54614	1	335234	5	NULL	NULL	0	NULL	p105			associates with					p50					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_1_556_s_373	12399470	A possible mode of sequestration could be binding to another cytoplasmic protein(s)  through the scaffold formed because of the association of p105 and p50 and the death  domain of p105.	transcription
55715	1	335234	7	NULL	NULL	0	NULL	p105			associate with			death domain		p50					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_1_556_s_373	12399470	A possible mode of sequestration could be binding to another cytoplasmic protein(s)  through the scaffold formed because of the association of p105 and p50 and the death  domain of p105.	transcription
54615	1	335235	5	NULL	NULL	0	NULL	NF-kappaB1 gene			encodes					p105					NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_8	9950430	The NF-kappaB1 gene encodes a larger precursor protein, p105, from which p50 is produced constitutively by proteasome-mediated removal of the p105 carboxy terminus 2-5.	transcription
54616	2	335235	5	NULL	NULL	0	NULL	p105			is a type of					large precursor protein					NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_8	9950430	The NF-kappaB1 gene encodes a larger precursor protein, p105, from which p50 is produced constitutively by proteasome-mediated removal of the p105 carboxy terminus 2-5.	transcription
54617	3	335235	5	NULL	NULL	0	NULL	p105		removal of	is mediated by			carboxy terminus		proteasome					NULL		NULL	NULL	NULL	NULL	gw60_nature_397_6717_363_s_8	9950430	The NF-kappaB1 gene encodes a larger precursor protein, p105, from which p50 is produced constitutively by proteasome-mediated removal of the p105 carboxy terminus 2-5.	transcription
54618	4	335235	5	NULL	NULL	0	NULL	statement 3			generates					p50					NULL		NULL	NULL	NULL	NULL	gw60_nature_397_6717_363_s_8	9950430	The NF-kappaB1 gene encodes a larger precursor protein, p105, from which p50 is produced constitutively by proteasome-mediated removal of the p105 carboxy terminus 2-5.	transcription
55716	1	335235	7	NULL	NULL	0	NULL	 NF-kappaB1 gene			encode					p105					NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_8	9950430	The NF-kappaB1 gene encodes a larger precursor protein, p105, from which p50 is produced constitutively by proteasome-mediated removal of the p105 carboxy terminus 2-5.	transcription
55717	2	335235	7	NULL	NULL	0	NULL	p105			is a type of					large precursor protein					NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_8	9950430	The NF-kappaB1 gene encodes a larger precursor protein, p105, from which p50 is produced constitutively by proteasome-mediated removal of the p105 carboxy terminus 2-5.	transcription
55718	3	335235	7	NULL	NULL	0	NULL	p50			produced from		constitutively			p105					NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_8	9950430	The NF-kappaB1 gene encodes a larger precursor protein, p105, from which p50 is produced constitutively by proteasome-mediated removal of the p105 carboxy terminus 2-5.	transcription
55719	4	335235	7	NULL	NULL	0	NULL	 proteasome			mediates					p105		removal of	carboxy terminus 2-5		NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_8	9950430	The NF-kappaB1 gene encodes a larger precursor protein, p105, from which p50 is produced constitutively by proteasome-mediated removal of the p105 carboxy terminus 2-5.	transcription
55720	5	335235	7	NULL	NULL	0	NULL	statement 3			occurs by					statement 4					NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_8	9950430	The NF-kappaB1 gene encodes a larger precursor protein, p105, from which p50 is produced constitutively by proteasome-mediated removal of the p105 carboxy terminus 2-5.	transcription
54619	1	335236	5	NULL	NULL	0	NULL	p105													NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_223	11158290	By physically interacting with the p105 mutants at an early step in the biogenesis of p105 and p50, unable to dissociate upon substrate phosphorylation due to lack of phosphorylation sites, it could hinder access of the proteasome or other processing components or affect p105 folding.	transcription
54620	1	335237	5	NULL	NULL	0	NULL	p50			associate with					p105					NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_326	10469655	Since a significant proportion of total p50 but less p65 is associated with p105, p105 plays a unique role in controlling p50 dimer activity (Ishikawa  et al., 1996  ).	transcription
54621	2	335237	5	NULL	NULL	0	NULL	p65			associate with					p105					NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_326	10469655	Since a significant proportion of total p50 but less p65 is associated with p105, p105 plays a unique role in controlling p50 dimer activity (Ishikawa  et al., 1996  ).	transcription
54622	3	335237	5	NULL	NULL	0	NULL	statement 1			is more than		significantly			statement 2					NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_326	10469655	Since a significant proportion of total p50 but less p65 is associated with p105, p105 plays a unique role in controlling p50 dimer activity (Ishikawa  et al., 1996  ).	transcription
54623	4	335237	5	NULL	NULL	0	NULL	p105			controls					p50 dimer		activity of			NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_326	10469655	Since a significant proportion of total p50 but less p65 is associated with p105, p105 plays a unique role in controlling p50 dimer activity (Ishikawa  et al., 1996  ).	transcription
55721	1	335237	7	NULL	NULL	0	NULL	 total p50		significant proportion of	associate with					p105					NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_326	10469655	Since a significant proportion of total p50 but less p65 is associated with p105, p105 plays a unique role in controlling p50 dimer activity (Ishikawa  et al., 1996  ).	transcription
55722	2	335237	7	NULL	NULL	0	NULL	p65			associate with					p105					NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_326	10469655	Since a significant proportion of total p50 but less p65 is associated with p105, p105 plays a unique role in controlling p50 dimer activity (Ishikawa  et al., 1996  ).	transcription
55724	3	335237	7	NULL	NULL	0	NULL	p105			controls					p50 dimer		activity of			NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_326	10469655	Since a significant proportion of total p50 but less p65 is associated with p105, p105 plays a unique role in controlling p50 dimer activity (Ishikawa  et al., 1996  ).	transcription
54628	1	335238	5	NULL	NULL	0	NULL	IKKbeta		expression of	increases					p50					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_318	11158290	We demonstrated that the expression of IKKbeta alone led to an increase in p50, but this effect is ascribed to IKKbeta-induced expression of p105, resulting in increased amounts of p50 produced by processing and loss of p105 by simultaneous IKKbeta-induced degradation.	transcription
54629	2	335238	5	NULL	NULL	0	NULL	p105		expression of	is induced by					IKKbeta					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_318	11158290	We demonstrated that the expression of IKKbeta alone led to an increase in p50, but this effect is ascribed to IKKbeta-induced expression of p105, resulting in increased amounts of p50 produced by processing and loss of p105 by simultaneous IKKbeta-induced degradation.	transcription
54630	3	335238	5	NULL	NULL	0	NULL	statement 2			ascribe					statement 1					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_318	11158290	We demonstrated that the expression of IKKbeta alone led to an increase in p50, but this effect is ascribed to IKKbeta-induced expression of p105, resulting in increased amounts of p50 produced by processing and loss of p105 by simultaneous IKKbeta-induced degradation.	transcription
54631	4	335238	5	NULL	NULL	0	NULL	statement 2			results in					p50		increased amounts of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_318	11158290	We demonstrated that the expression of IKKbeta alone led to an increase in p50, but this effect is ascribed to IKKbeta-induced expression of p105, resulting in increased amounts of p50 produced by processing and loss of p105 by simultaneous IKKbeta-induced degradation.	transcription
54632	5	335238	5	NULL	NULL	0	NULL	p50			is produced by					p105		processing of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_318	11158290	We demonstrated that the expression of IKKbeta alone led to an increase in p50, but this effect is ascribed to IKKbeta-induced expression of p105, resulting in increased amounts of p50 produced by processing and loss of p105 by simultaneous IKKbeta-induced degradation.	transcription
54633	6	335238	5	NULL	NULL	0	NULL	p50			is produced by					p105		loss of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_318	11158290	We demonstrated that the expression of IKKbeta alone led to an increase in p50, but this effect is ascribed to IKKbeta-induced expression of p105, resulting in increased amounts of p50 produced by processing and loss of p105 by simultaneous IKKbeta-induced degradation.	transcription
54634	7	335238	5	NULL	NULL	0	NULL	statement 5			occurs simultaneously with					statement 6					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_318	11158290	We demonstrated that the expression of IKKbeta alone led to an increase in p50, but this effect is ascribed to IKKbeta-induced expression of p105, resulting in increased amounts of p50 produced by processing and loss of p105 by simultaneous IKKbeta-induced degradation.	transcription
54635	8	335238	5	NULL	NULL	0	NULL	IKKbeta			induce					degradation					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_318	11158290	We demonstrated that the expression of IKKbeta alone led to an increase in p50, but this effect is ascribed to IKKbeta-induced expression of p105, resulting in increased amounts of p50 produced by processing and loss of p105 by simultaneous IKKbeta-induced degradation.	transcription
54636	9	335238	5	NULL	NULL	0	NULL	statement 8			occurs simultaneously with					statement 7					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_318	11158290	We demonstrated that the expression of IKKbeta alone led to an increase in p50, but this effect is ascribed to IKKbeta-induced expression of p105, resulting in increased amounts of p50 produced by processing and loss of p105 by simultaneous IKKbeta-induced degradation.	transcription
55725	1	335238	7	NULL	NULL	0	NULL	IKKbeta			induce					p105		expression of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_318	11158290	We demonstrated that the expression of IKKbeta alone led to an increase in p50, but this effect is ascribed to IKKbeta-induced expression of p105, resulting in increased amounts of p50 produced by processing and loss of p105 by simultaneous IKKbeta-induced degradation.	transcription
55726	2	335238	7	NULL	NULL	0	NULL	statement 1			result in					p50		increased amounts of 			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_318	11158290	We demonstrated that the expression of IKKbeta alone led to an increase in p50, but this effect is ascribed to IKKbeta-induced expression of p105, resulting in increased amounts of p50 produced by processing and loss of p105 by simultaneous IKKbeta-induced degradation.	transcription
55727	3	335238	7	NULL	NULL	0	NULL	p50			produced by					p105		processing of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_318	11158290	We demonstrated that the expression of IKKbeta alone led to an increase in p50, but this effect is ascribed to IKKbeta-induced expression of p105, resulting in increased amounts of p50 produced by processing and loss of p105 by simultaneous IKKbeta-induced degradation.	transcription
55728	5	335238	7	NULL	NULL	0	NULL	p50			produced by					p105		loss of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_318	11158290	We demonstrated that the expression of IKKbeta alone led to an increase in p50, but this effect is ascribed to IKKbeta-induced expression of p105, resulting in increased amounts of p50 produced by processing and loss of p105 by simultaneous IKKbeta-induced degradation.	transcription
55729	4	335238	7	NULL	NULL	0	NULL	IKKbeta			induce					p105		degradation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_318	11158290	We demonstrated that the expression of IKKbeta alone led to an increase in p50, but this effect is ascribed to IKKbeta-induced expression of p105, resulting in increased amounts of p50 produced by processing and loss of p105 by simultaneous IKKbeta-induced degradation.	transcription
55730	6	335238	7	NULL	NULL	0	NULL	statement 4			leads to					statement 5					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_318	11158290	We demonstrated that the expression of IKKbeta alone led to an increase in p50, but this effect is ascribed to IKKbeta-induced expression of p105, resulting in increased amounts of p50 produced by processing and loss of p105 by simultaneous IKKbeta-induced degradation.	transcription
54637	1	335239	5	NULL	NULL	0	NULL	p50			is synthesized from		de novo			p105					NULL	tolerant CD4+ T cells 	0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8460_s_214	14668329	Thus, the increased expression of p50 in tolerant CD4+ T cells could reflect  de novo synthesis of p50 from p105 following tolerance induction.	transcription
55731	1	335239	7	NULL	NULL	0	NULL	p50			produced by					p105		de novo synthesis of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8460_s_214	14668329	Thus, the increased expression of p50 in tolerant CD4+ T cells could reflect  de novo synthesis of p50 from p105 following tolerance induction.	transcription
55732	2	335239	7	NULL	NULL	0	NULL	p50		increased expression of	reflect					statement 1					NULL	tolerant CD4+ T cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_8460_s_214	14668329	Thus, the increased expression of p50 in tolerant CD4+ T cells could reflect  de novo synthesis of p50 from p105 following tolerance induction.	transcription
55733	3	335239	7	NULL	NULL	0	NULL	statement 1			occurs following					tolerance		induction of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8460_s_214	14668329	Thus, the increased expression of p50 in tolerant CD4+ T cells could reflect  de novo synthesis of p50 from p105 following tolerance induction.	transcription
54638	1	335240	5	NULL	NULL	0	NULL	p50		cotranslational folding of	regulates		might			p50		primary ratio of			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_17_4712_s_35	10970863	In our previous work, we proposed that cotranslational folding of p50 might regulate the primary ratio of p50 and p105 ( Lin   et al., 1998).	transcription
54639	2	335240	5	NULL	NULL	0	NULL	p50		cotranslational folding of	regulates		might			p105		primary ratio of			NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_35	10970863	In our previous work, we proposed that cotranslational folding of p50 might regulate the primary ratio of p50 and p105 ( Lin   et al., 1998).	transcription
54640	3	335240	5	NULL	NULL	0	NULL	statement 1			occurs along with					statement 2					NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_35	10970863	In our previous work, we proposed that cotranslational folding of p50 might regulate the primary ratio of p50 and p105 ( Lin   et al., 1998).	transcription
55734	1	335240	7	NULL	NULL	0	NULL	p50		cotranslational folding of	regulate		might			p50		primary ratio of			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_17_4712_s_35	10970863	In our previous work, we proposed that cotranslational folding of p50 might regulate the primary ratio of p50 and p105 ( Lin   et al., 1998).	transcription
55735	2	335240	7	NULL	NULL	0	NULL	p50		cotranslational folding of	regulate		might			p105		primary ratio of			NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_35	10970863	In our previous work, we proposed that cotranslational folding of p50 might regulate the primary ratio of p50 and p105 ( Lin   et al., 1998).	transcription
55736	3	335240	7	NULL	NULL	0	NULL	statement 1			occur along with					statement 2					NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_35	10970863	In our previous work, we proposed that cotranslational folding of p50 might regulate the primary ratio of p50 and p105 ( Lin   et al., 1998).	transcription
54641	1	335241	5	NULL	NULL	0	NULL	p105			is substituted with			ankyrin repeats		DHFR					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_201	11350967	Panel B, substitution of four ankyrin repeats with DHFR abrogates the ability of p50 to inhibit processing of p105 and does not prevent nuclear translocation of free p50.	transcription
54642	2	335241	5	NULL	NULL	0	NULL	p50			inhibits					p105		processing of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_201	11350967	Panel B, substitution of four ankyrin repeats with DHFR abrogates the ability of p50 to inhibit processing of p105 and does not prevent nuclear translocation of free p50.	transcription
54643	3	335241	5	NULL	NULL	0	NULL	statement 1			abrogates					statement 2					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_201	11350967	Panel B, substitution of four ankyrin repeats with DHFR abrogates the ability of p50 to inhibit processing of p105 and does not prevent nuclear translocation of free p50.	transcription
54644	4	335241	5	NULL	NULL	0	NULL	p50		free	is translocated to					nucleus					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_201	11350967	Panel B, substitution of four ankyrin repeats with DHFR abrogates the ability of p50 to inhibit processing of p105 and does not prevent nuclear translocation of free p50.	transcription
54645	5	335241	5	NULL	NULL	0	NULL	statement 1			does not prevent					statement 4					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_201	11350967	Panel B, substitution of four ankyrin repeats with DHFR abrogates the ability of p50 to inhibit processing of p105 and does not prevent nuclear translocation of free p50.	transcription
55737	1	335241	7	NULL	NULL	0	NULL	p50			inhibit					p105		processing of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_201	11350967	Panel B, substitution of four ankyrin repeats with DHFR abrogates the ability of p50 to inhibit processing of p105 and does not prevent nuclear translocation of free p50.	transcription
55738	2	335241	7	NULL	NULL	0	NULL				substituted with			 four ankyrin repeats		DHFR					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_201	11350967	Panel B, substitution of four ankyrin repeats with DHFR abrogates the ability of p50 to inhibit processing of p105 and does not prevent nuclear translocation of free p50.	transcription
55739	3	335241	7	NULL	NULL	0	NULL	statement 2			abrogates					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_201	11350967	Panel B, substitution of four ankyrin repeats with DHFR abrogates the ability of p50 to inhibit processing of p105 and does not prevent nuclear translocation of free p50.	transcription
55740	4	335241	7	NULL	NULL	0	NULL	statement 2			does not prevent					p50		nuclear translocation of free			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_201	11350967	Panel B, substitution of four ankyrin repeats with DHFR abrogates the ability of p50 to inhibit processing of p105 and does not prevent nuclear translocation of free p50.	transcription
54646	1	335242	5	NULL	NULL	0	NULL	p50			is generated from					p105					NULL	T2 cell extracts	0	NULL	NULL	NULL	gw60_jbiolchem_275_7_5238_s_196	10671572	Impaired Processing of p50 in T2 Cell Extracts-- The generation of p50 from p105 is mediated by the ubiquitin-proteasome processing pathway ( 28,  44,  46,  61).	transcription
54647	2	335242	5	NULL	NULL	0	NULL	statement 1			is mediated by					ubiquitin-proteasome processing pathway					NULL	T2 cell extracts	0	NULL	NULL	NULL	gw60_jbiolchem_275_7_5238_s_196	10671572	Impaired Processing of p50 in T2 Cell Extracts-- The generation of p50 from p105 is mediated by the ubiquitin-proteasome processing pathway ( 28,  44,  46,  61).	transcription
55741	1	335242	7	NULL	NULL	0	NULL	 p50 			generated from					p105					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_7_5238_s_196	10671572	Impaired Processing of p50 in T2 Cell Extracts-- The generation of p50 from p105 is mediated by the ubiquitin-proteasome processing pathway ( 28,  44,  46,  61).	transcription
55742	2	335242	7	NULL	NULL	0	NULL	statement 1			mediated by					ubiquitin-proteasome processing pathway					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_7_5238_s_196	10671572	Impaired Processing of p50 in T2 Cell Extracts-- The generation of p50 from p105 is mediated by the ubiquitin-proteasome processing pathway ( 28,  44,  46,  61).	transcription
55743	3	335242	7	NULL	NULL	0	NULL	p50		processing of	impaired in					T2 Cell Extracts					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_7_5238_s_196	10671572	Impaired Processing of p50 in T2 Cell Extracts-- The generation of p50 from p105 is mediated by the ubiquitin-proteasome processing pathway ( 28,  44,  46,  61).	transcription
54648	1	335243	5	NULL	NULL	0	NULL	p105			is processed to					p50					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_545_s_147	15020252	This is because  degradation of I B and processing of p105 to p50 are mediated by the ubiquitin/proteasome  system [ 3.	transcription
54649	2	335243	5	NULL	NULL	0	NULL	ubiquitin/proteasome system			mediates					statement 1					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_545_s_147	15020252	This is because  degradation of I B and processing of p105 to p50 are mediated by the ubiquitin/proteasome  system [ 3.	transcription
54650	3	335243	5	NULL	NULL	0	NULL	ubiquitin/proteasome system			mediates					I B		degradation of			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_545_s_147	15020252	This is because  degradation of I B and processing of p105 to p50 are mediated by the ubiquitin/proteasome  system [ 3.	transcription
55744	1	335243	7	NULL	NULL	0	NULL	I B		 degradation of	is mediated by					ubiquitin/proteasome system					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_545_s_147	15020252	This is because  degradation of I B and processing of p105 to p50 are mediated by the ubiquitin/proteasome  system [ 3.	transcription
55745	2	335243	7	NULL	NULL	0	NULL	p105			processed to					p50					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_545_s_147	15020252	This is because  degradation of I B and processing of p105 to p50 are mediated by the ubiquitin/proteasome  system [ 3.	transcription
55746	3	335243	7	NULL	NULL	0	NULL	statement 2			mediated by					ubiquitin/proteasome system					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_316_2_545_s_147	15020252	This is because  degradation of I B and processing of p105 to p50 are mediated by the ubiquitin/proteasome  system [ 3.	transcription
54651	1	335244	5	NULL	NULL	0	NULL	GSK-3beta			regulates					NF-kappaB					NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_23	16192643	GSK-3beta regulates NF-kappaB by phosphorylating its p65 transactivation subunit   and by phosphorylating and stabilizing p105, the precursor of its p50 subunit.	transcription
54652	2	335244	5	NULL	NULL	0	NULL	GSK-3beta			phosphorylates					NF-kappaB			p65 subuint		NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_23	16192643	GSK-3beta regulates NF-kappaB by phosphorylating its p65 transactivation subunit   and by phosphorylating and stabilizing p105, the precursor of its p50 subunit.	transcription
54653	3	335244	5	NULL	NULL	0	NULL	statement 2			leads to					statement 1					NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_23	16192643	GSK-3beta regulates NF-kappaB by phosphorylating its p65 transactivation subunit   and by phosphorylating and stabilizing p105, the precursor of its p50 subunit.	transcription
54654	4	335244	5	NULL	NULL	0	NULL	NF-kappaB			is a type of			p65 subunit		transactivation subunit					NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_23	16192643	GSK-3beta regulates NF-kappaB by phosphorylating its p65 transactivation subunit   and by phosphorylating and stabilizing p105, the precursor of its p50 subunit.	transcription
54655	5	335244	5	NULL	NULL	0	NULL	p105			is a precursor of								p50 subunit		NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_23	16192643	GSK-3beta regulates NF-kappaB by phosphorylating its p65 transactivation subunit   and by phosphorylating and stabilizing p105, the precursor of its p50 subunit.	transcription
54656	6	335244	5	NULL	NULL	0	NULL	GSK-3beta			stabilize					p105					NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_23	16192643	GSK-3beta regulates NF-kappaB by phosphorylating its p65 transactivation subunit   and by phosphorylating and stabilizing p105, the precursor of its p50 subunit.	transcription
55747	1	335244	7	NULL	NULL	0	NULL	GSK-3beta			regulates					NF-kappaB					NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_23	16192643	GSK-3beta regulates NF-kappaB by phosphorylating its p65 transactivation subunit   and by phosphorylating and stabilizing p105, the precursor of its p50 subunit.	transcription
55748	2	335244	7	NULL	NULL	0	NULL	statement 1			occur by					p65		phosphorylation of	transactivation subunit		NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_23	16192643	GSK-3beta regulates NF-kappaB by phosphorylating its p65 transactivation subunit   and by phosphorylating and stabilizing p105, the precursor of its p50 subunit.	transcription
55749	3	335244	7	NULL	NULL	0	NULL	statement 1			occur by					p105		phosphorylating;;stabilizing			NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_23	16192643	GSK-3beta regulates NF-kappaB by phosphorylating its p65 transactivation subunit   and by phosphorylating and stabilizing p105, the precursor of its p50 subunit.	transcription
55750	4	335244	7	NULL	NULL	0	NULL	p105			is a precursor of					p50 subunit					NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_23	16192643	GSK-3beta regulates NF-kappaB by phosphorylating its p65 transactivation subunit   and by phosphorylating and stabilizing p105, the precursor of its p50 subunit.	transcription
54657	1	335245	5	NULL	NULL	0	NULL	p105			is a regulator of		negative			TPL-2					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_12_5235_s_26	15169888	Thus, in addition to its roles as a precursor for p50 and an IkappaB, p105 functions as a negative regulator of TPL-2.	transcription
54658	2	335245	5	NULL	NULL	0	NULL	p105			is a precursor of					p50					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_12_5235_s_26	15169888	Thus, in addition to its roles as a precursor for p50 and an IkappaB, p105 functions as a negative regulator of TPL-2.	transcription
54659	3	335245	5	NULL	NULL	0	NULL	p105			is a precursor of					IkappaB					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_12_5235_s_26	15169888	Thus, in addition to its roles as a precursor for p50 and an IkappaB, p105 functions as a negative regulator of TPL-2.	transcription
55751	1	335245	7	NULL	NULL	0	NULL	p105			is a precursor of					p50					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_12_5235_s_26	15169888	Thus, in addition to its roles as a precursor for p50 and an IkappaB, p105 functions as a negative regulator of TPL-2.	transcription
55752	2	335245	7	NULL	NULL	0	NULL	p105			is a precursor of					IkappaB					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_12_5235_s_26	15169888	Thus, in addition to its roles as a precursor for p50 and an IkappaB, p105 functions as a negative regulator of TPL-2.	transcription
55753	3	335245	7	NULL	NULL	0	NULL	p105			regulates		negatively			 TPL-2					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_12_5235_s_26	15169888	Thus, in addition to its roles as a precursor for p50 and an IkappaB, p105 functions as a negative regulator of TPL-2.	transcription
54660	1	335246	5	NULL	NULL	0	NULL	nfkb1 gene			encodes					p50					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_2	12807880	he NF-kappaB transcription factor p50 and the Rel protein-specific  transcription inhibitor p105 are both encoded by the  nfkb1 gene.	transcription
54661	2	335246	5	NULL	NULL	0	NULL	nfkb1 gene			encodes					p105					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_2	12807880	he NF-kappaB transcription factor p50 and the Rel protein-specific  transcription inhibitor p105 are both encoded by the  nfkb1 gene.	transcription
54662	3	335246	5	NULL	NULL	0	NULL	p105			is a type of					Rel protein-specific transcription inhibitor					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_2	12807880	he NF-kappaB transcription factor p50 and the Rel protein-specific  transcription inhibitor p105 are both encoded by the  nfkb1 gene.	transcription
54663	4	335246	5	NULL	NULL	0	NULL	p50			is a type of					NF-kappaB transcription factor					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_2	12807880	he NF-kappaB transcription factor p50 and the Rel protein-specific  transcription inhibitor p105 are both encoded by the  nfkb1 gene.	transcription
55754	1	335246	7	NULL	NULL	0	NULL	 nfkb1 gene			encode					p50					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_2	12807880	he NF-kappaB transcription factor p50 and the Rel protein-specific  transcription inhibitor p105 are both encoded by the  nfkb1 gene.	transcription
55755	2	335246	7	NULL	NULL	0	NULL	 nfkb1 gene			encode					p105					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_2	12807880	he NF-kappaB transcription factor p50 and the Rel protein-specific  transcription inhibitor p105 are both encoded by the  nfkb1 gene.	transcription
55756	3	335246	7	NULL	NULL	0	NULL	p50			is a type of					NF-kappaB transcription factor					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_2	12807880	he NF-kappaB transcription factor p50 and the Rel protein-specific  transcription inhibitor p105 are both encoded by the  nfkb1 gene.	transcription
55757	4	335246	7	NULL	NULL	0	NULL	p105			is a type of					Rel protein-specific transcription inhibitor					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_2	12807880	he NF-kappaB transcription factor p50 and the Rel protein-specific  transcription inhibitor p105 are both encoded by the  nfkb1 gene.	transcription
54664	1	335247	5	NULL	NULL	0	NULL	SCFbetaTrCP complex			bind					p105					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_20	12807880	The binding of the SCFbetaTrCP complex to p105 was  originally attributed to enhancement of p50 generation upon stimulation  ( ,   ).	transcription
55758	1	335247	7	NULL	NULL	0	NULL	SCFbetaTrCP complex			bind					p105					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_20	12807880	The binding of the SCFbetaTrCP complex to p105 was  originally attributed to enhancement of p50 generation upon stimulation  ( ,   ).	transcription
55759	2	335247	7	NULL	NULL	0	NULL	statement 1			occurs upon					p50		enhancement of;; generation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_20	12807880	The binding of the SCFbetaTrCP complex to p105 was  originally attributed to enhancement of p50 generation upon stimulation  ( ,   ).	transcription
55760	3	335247	7	NULL	NULL	0	NULL	statement 2			occurs upon					stimulation					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_20	12807880	The binding of the SCFbetaTrCP complex to p105 was  originally attributed to enhancement of p50 generation upon stimulation  ( ,   ).	transcription
54665	1	335248	5	NULL	NULL	0	NULL	p105		deletion mutant	does not effect			C terminus		p50		level of			NULL	resting cells	0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_184	12807880	B, deletion of the C terminus of p105 does not affect p50 level in  resting cells.	transcription
55761	1	335248	7	NULL	NULL	0	NULL	p105		deletion of	does not affect			C terminus		p50		level of			NULL	resting cells	0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_184	12807880	B, deletion of the C terminus of p105 does not affect p50 level in  resting cells.	transcription
54666	1	335249	5	NULL	NULL	0	NULL	TNF-alpha			fails to induce					p105		degradation of			NULL	GSK-3beta - / - fibroblasts	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_41_39583_s_186	12871932	On the contrary, in  GSK-3beta - / -  fibroblasts p50 appears to accumulate significantly in the control chase, while TNF-alpha fails to induce p105 degradation.	transcription
55762	1	335249	7	NULL	NULL	0	NULL	TNF-alpha			does not induce					p105		degradation of			NULL	GSK-3beta - / - fibroblasts 	0	NULL	NULL	NULL	gw70_jbiolchem_278_41_39583_s_186	12871932	On the contrary, in  GSK-3beta - / -  fibroblasts p50 appears to accumulate significantly in the control chase, while TNF-alpha fails to induce p105 degradation.	transcription
54678	1	335250	5	NULL	NULL	0	NULL	p105			is associated with		predominantly			p50					NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_322	10469655	Depending on relative expression levels, p105 is associated predominantly with p50, generated by constitutive processing, or with other NF-kappaB subunits.	transcription
54679	2	335250	5	NULL	NULL	0	NULL	p50			is generated by					p105		constitutive processing of			NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_322	10469655	Depending on relative expression levels, p105 is associated predominantly with p50, generated by constitutive processing, or with other NF-kappaB subunits.	transcription
54680	3	335250	5	NULL	NULL	0	NULL	p105			is associated with					NF-kappaB subunits					NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_322	10469655	Depending on relative expression levels, p105 is associated predominantly with p50, generated by constitutive processing, or with other NF-kappaB subunits.	transcription
55763	1	335250	7	NULL	NULL	0	NULL	p105			associate with		predominantly			p50					NULL		NULL	NULL	NULL	NULL	gw60_embo_18_17_4766_s_322	10469655	Depending on relative expression levels, p105 is associated predominantly with p50, generated by constitutive processing, or with other NF-kappaB subunits.	transcription
55764	2	335250	7	NULL	NULL	0	NULL	p50			generated by					constitutive processing					NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_322	10469655	Depending on relative expression levels, p105 is associated predominantly with p50, generated by constitutive processing, or with other NF-kappaB subunits.	transcription
55765	3	335250	7	NULL	NULL	0	NULL	p105			associate with					NF-kappaB 			subunits		NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_322	10469655	Depending on relative expression levels, p105 is associated predominantly with p50, generated by constitutive processing, or with other NF-kappaB subunits.	transcription
54681	1	335251	5	NULL	NULL	0	NULL	p105 gene		expression of	is regulated by					NF-kappaB					NULL		0	NULL	NULL	NULL	gw60_genesdev_15_18_2321_s_214	11562344	Regulated processing is difficult to demonstrate for p50 because expression of the p105 gene is itself regulated by NF-kappaB.	transcription
55766	1	335251	7	NULL	NULL	0	NULL	 NF-kappaB			regulates					p105 gene		expression of			NULL		0	NULL	NULL	NULL	gw60_genesdev_15_18_2321_s_214	11562344	Regulated processing is difficult to demonstrate for p50 because expression of the p105 gene is itself regulated by NF-kappaB.	transcription
54682	1	335252	5	NULL	NULL	0	NULL	p50			corresponds to					p105			N terminus		NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_3	9529257	p50  corresponds to the N terminus of p105 and with p65 (RelA) forms the  prototypical NF- B transcription factor complex.	transcription
54683	2	335252	5	NULL	NULL	0	NULL	p65			is a synonym of					RelA					NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_3	9529257	p50  corresponds to the N terminus of p105 and with p65 (RelA) forms the  prototypical NF- B transcription factor complex.	transcription
54684	3	335252	5	NULL	NULL	0	NULL	p65			forms					NF- B transcription factor complex		prototypical			NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_3	9529257	p50  corresponds to the N terminus of p105 and with p65 (RelA) forms the  prototypical NF- B transcription factor complex.	transcription
55767	1	335252	7	NULL	NULL	0	NULL	p50			corresponds to					p105			N terminus		NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_3	9529257	p50  corresponds to the N terminus of p105 and with p65 (RelA) forms the  prototypical NF- B transcription factor complex.	transcription
55768	2	335252	7	NULL	NULL	0	NULL	p50			associate with					p65					NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_3	9529257	p50  corresponds to the N terminus of p105 and with p65 (RelA) forms the  prototypical NF- B transcription factor complex.	transcription
55769	3	335252	7	NULL	NULL	0	NULL	statement 2			forms					NF- B transcription factor complex		prototypical			NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_3	9529257	p50  corresponds to the N terminus of p105 and with p65 (RelA) forms the  prototypical NF- B transcription factor complex.	transcription
54685	1	335253	5	NULL	NULL	0	NULL	NF- B			is a type of					transcription factor					NULL		0	NULL	NULL	NULL	gw60_molcell_7_3_627_s_30	11463387	The transcription factor NF- B subunit p50 is produced by partial proteolysis of the p105 precursor protein by the proteasome.	transcription
54686	2	335253	5	NULL	NULL	0	NULL	p105 precursor protein			undergoes					proteolysis		partial			NULL		0	NULL	NULL	NULL	gw60_molcell_7_3_627_s_30	11463387	The transcription factor NF- B subunit p50 is produced by partial proteolysis of the p105 precursor protein by the proteasome.	transcription
54687	3	335253	5	NULL	NULL	0	NULL	proteasome			is required for					statement 1					NULL		0	NULL	NULL	NULL	gw60_molcell_7_3_627_s_30	11463387	The transcription factor NF- B subunit p50 is produced by partial proteolysis of the p105 precursor protein by the proteasome.	transcription
54689	4	335253	5	NULL	NULL	0	NULL	statement 2			produces					NF- B			p50 subunit		NULL		0	NULL	NULL	NULL	gw60_molcell_7_3_627_s_30	11463387	The transcription factor NF- B subunit p50 is produced by partial proteolysis of the p105 precursor protein by the proteasome.	transcription
55770	1	335253	7	NULL	NULL	0	NULL	p50 			produced by					p105 precursor protein		partial proteolysis of 			NULL		0	NULL	NULL	NULL	gw60_molcell_7_3_627_s_30	11463387	The transcription factor NF- B subunit p50 is produced by partial proteolysis of the p105 precursor protein by the proteasome.	transcription
55771	2	335253	7	NULL	NULL	0	NULL	statement 1			occur by					proteasome					NULL		0	NULL	NULL	NULL	gw60_molcell_7_3_627_s_30	11463387	The transcription factor NF- B subunit p50 is produced by partial proteolysis of the p105 precursor protein by the proteasome.	transcription
55772	3	335253	7	NULL	NULL	0	NULL	 p50			is subunit of					NF- B transcription factor					NULL		0	NULL	NULL	NULL	gw60_molcell_7_3_627_s_30	11463387	The transcription factor NF- B subunit p50 is produced by partial proteolysis of the p105 precursor protein by the proteasome.	transcription
54690	1	335254	5	NULL	NULL	0	NULL	TNF-alpha			induces					p105		degradation of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_42	11158290	TNF-alpha-induced p105 degradation rapidly releases p105-bound p50, which is detected in the nucleus as dimers complexed with Bcl-3 ( 13).	transcription
54691	3	335254	5	NULL	NULL	0	NULL	statement 1			releases		rapidly			statement 2					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_42	11158290	TNF-alpha-induced p105 degradation rapidly releases p105-bound p50, which is detected in the nucleus as dimers complexed with Bcl-3 ( 13).	transcription
54692	2	335254	5	NULL	NULL	0	NULL	p50			bind					p105					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_42	11158290	TNF-alpha-induced p105 degradation rapidly releases p105-bound p50, which is detected in the nucleus as dimers complexed with Bcl-3 ( 13).	transcription
54693	4	335254	5	NULL	NULL	0	NULL	statement 2			complexes with					Bcl-3					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_42	11158290	TNF-alpha-induced p105 degradation rapidly releases p105-bound p50, which is detected in the nucleus as dimers complexed with Bcl-3 ( 13).	transcription
55773	1	335254	7	NULL	NULL	0	NULL	TNF-alpha			induce					p105		degradation of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_42	11158290	TNF-alpha-induced p105 degradation rapidly releases p105-bound p50, which is detected in the nucleus as dimers complexed with Bcl-3 ( 13).	transcription
55774	2	335254	7	NULL	NULL	0	NULL	p50			bind					p105					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_42	11158290	TNF-alpha-induced p105 degradation rapidly releases p105-bound p50, which is detected in the nucleus as dimers complexed with Bcl-3 ( 13).	transcription
55775	3	335254	7	NULL	NULL	0	NULL	statement 1			release		rapidly			statement 2					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_42	11158290	TNF-alpha-induced p105 degradation rapidly releases p105-bound p50, which is detected in the nucleus as dimers complexed with Bcl-3 ( 13).	transcription
55776	4	335254	7	NULL	NULL	0	NULL	statement 2			complexed with					Bcl-3					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_42	11158290	TNF-alpha-induced p105 degradation rapidly releases p105-bound p50, which is detected in the nucleus as dimers complexed with Bcl-3 ( 13).	transcription
55777	5	335254	7	NULL	NULL	0	NULL	statement 4			detected as					dimers					NULL	nucleus	0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_42	11158290	TNF-alpha-induced p105 degradation rapidly releases p105-bound p50, which is detected in the nucleus as dimers complexed with Bcl-3 ( 13).	transcription
54694	1	335255	5	NULL	NULL	0	NULL	p105			is a regulator of		negative			TPL-2					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_14_4739_s_9	12832462	Thus, in addition to its role as a precursor for p50 and cytoplasmic inhibitor of NF-kappaB, p105 is a negative regulator of TPL-2.	transcription
54695	2	335255	5	NULL	NULL	0	NULL	p105			is a precursor for					p50					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_14_4739_s_9	12832462	Thus, in addition to its role as a precursor for p50 and cytoplasmic inhibitor of NF-kappaB, p105 is a negative regulator of TPL-2.	transcription
54696	3	335255	5	NULL	NULL	0	NULL	p105			is an inhibitor of					NF-kappaB					NULL	cytoplasm	0	NULL	NULL	NULL	gw60_molcellbiol_23_14_4739_s_9	12832462	Thus, in addition to its role as a precursor for p50 and cytoplasmic inhibitor of NF-kappaB, p105 is a negative regulator of TPL-2.	transcription
55778	1	335255	7	NULL	NULL	0	NULL	p105			is a precursor of					p50					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_14_4739_s_9	12832462	Thus, in addition to its role as a precursor for p50 and cytoplasmic inhibitor of NF-kappaB, p105 is a negative regulator of TPL-2.	transcription
55779	2	335255	7	NULL	NULL	0	NULL	p105			is a precursor of					NF-kappaB					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_14_4739_s_9	12832462	Thus, in addition to its role as a precursor for p50 and cytoplasmic inhibitor of NF-kappaB, p105 is a negative regulator of TPL-2.	transcription
55780	3	335255	7	NULL	NULL	0	NULL	p105			regulates		negatively			TPL-2					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_14_4739_s_9	12832462	Thus, in addition to its role as a precursor for p50 and cytoplasmic inhibitor of NF-kappaB, p105 is a negative regulator of TPL-2.	transcription
55781	4	335255	7	NULL	NULL	0	NULL	NF-kappaB			is a type of					cytoplasmic inhibitor					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_14_4739_s_9	12832462	Thus, in addition to its role as a precursor for p50 and cytoplasmic inhibitor of NF-kappaB, p105 is a negative regulator of TPL-2.	transcription
54697	1	335256	5	NULL	NULL	0	NULL	NF-kappaB1			is a regulator of		negative	p105		TPL-2					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_14_4739_s_363	12832462	NF-kappaB1 p105 is therefore a negative regulator of TPL-2 MEK kinase, in addition to its functions as a precursor for p50 and an IkappaB protein ( 18).	transcription
54698	2	335256	5	NULL	NULL	0	NULL	TPL-2			is a type of					MEK kinase					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_14_4739_s_363	12832462	NF-kappaB1 p105 is therefore a negative regulator of TPL-2 MEK kinase, in addition to its functions as a precursor for p50 and an IkappaB protein ( 18).	transcription
54699	3	335256	5	NULL	NULL	0	NULL	NF-kappaB1			function as			p105		p50		precursor of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_14_4739_s_363	12832462	NF-kappaB1 p105 is therefore a negative regulator of TPL-2 MEK kinase, in addition to its functions as a precursor for p50 and an IkappaB protein ( 18).	transcription
54700	4	335256	5	NULL	NULL	0	NULL	NF-kappaB1			is a type of			p105		IkappaB protein					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_14_4739_s_363	12832462	NF-kappaB1 p105 is therefore a negative regulator of TPL-2 MEK kinase, in addition to its functions as a precursor for p50 and an IkappaB protein ( 18).	transcription
55782	1	335256	7	NULL	NULL	0	NULL	NF-kappaB1 p105			regulates		negatively			TPL-2 MEK kinase					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_14_4739_s_363	12832462	NF-kappaB1 p105 is therefore a negative regulator of TPL-2 MEK kinase, in addition to its functions as a precursor for p50 and an IkappaB protein ( 18).	transcription
55783	2	335256	7	NULL	NULL	0	NULL	NF-kappaB1 p105			is a precursor of					p50 dimer					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_14_4739_s_363	12832462	NF-kappaB1 p105 is therefore a negative regulator of TPL-2 MEK kinase, in addition to its functions as a precursor for p50 and an IkappaB protein ( 18).	transcription
55784	3	335256	7	NULL	NULL	0	NULL	NF-kappaB1 p105			is a precursor of					IkappaB protein					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_14_4739_s_363	12832462	NF-kappaB1 p105 is therefore a negative regulator of TPL-2 MEK kinase, in addition to its functions as a precursor for p50 and an IkappaB protein ( 18).	transcription
54701	1	335257	5	NULL	NULL	0	NULL	NF-kappaB1			function as			p105		NF-kappaB1		precursor of	p50		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_1_402_s_2	12482991	F-kappaB1 p105 functions both as a precursor of NF-kappaB1 p50 and as a cytoplasmic inhibitor of NF-kappaB.	transcription
54702	2	335257	5	NULL	NULL	0	NULL	NF-kappaB1			is an inhibitor of			p105		NF-kappaB					NULL	cytoplasm	0	NULL	NULL	NULL	gw60_molcellbiol_23_1_402_s_2	12482991	F-kappaB1 p105 functions both as a precursor of NF-kappaB1 p50 and as a cytoplasmic inhibitor of NF-kappaB.	transcription
55785	1	335257	7	NULL	NULL	0	NULL	F-kappaB1 p105			is a precursor of					NF-kappaB1 p50					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_1_402_s_2	12482991	F-kappaB1 p105 functions both as a precursor of NF-kappaB1 p50 and as a cytoplasmic inhibitor of NF-kappaB.	transcription
55786	2	335257	7	NULL	NULL	0	NULL	F-kappaB1 p105			is a precursor of					NF-kappaB					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_1_402_s_2	12482991	F-kappaB1 p105 functions both as a precursor of NF-kappaB1 p50 and as a cytoplasmic inhibitor of NF-kappaB.	transcription
55787	3	335257	7	NULL	NULL	0	NULL	NF-kappaB			is a type of					cytoplasmic inhibitor					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_1_402_s_2	12482991	F-kappaB1 p105 functions both as a precursor of NF-kappaB1 p50 and as a cytoplasmic inhibitor of NF-kappaB.	transcription
55788	1	335258	7	NULL	NULL	0	NULL	TNF			stimulate					LNCaP cells					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_13_11116_s_178	11799112	D, p50 activity was measured as a function of p105 processing in TNF-stimulated LNCaP cells expressing either GFP or PTEN.	transcription
55789	2	335258	7	NULL	NULL	0	NULL	statement 1			express					GFP					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_13_11116_s_178	11799112	D, p50 activity was measured as a function of p105 processing in TNF-stimulated LNCaP cells expressing either GFP or PTEN.	transcription
55790	3	335258	7	NULL	NULL	0	NULL	statement 1			express					PTEN					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_13_11116_s_178	11799112	D, p50 activity was measured as a function of p105 processing in TNF-stimulated LNCaP cells expressing either GFP or PTEN.	transcription
55791	4	335258	7	NULL	NULL	0	NULL	statement 2			is an alternative to					statement 3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_13_11116_s_178	11799112	D, p50 activity was measured as a function of p105 processing in TNF-stimulated LNCaP cells expressing either GFP or PTEN.	transcription
54703	1	335259	5	NULL	NULL	0	NULL	p105		cleavage of	is mediated by					proteasome					NULL	T2 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_7_5238_s_231	10671572	Overall, these data suggest that the defect in p50 generation in T2 cells is due to a failure of proteasome-mediated cleavage of p105.	transcription
54704	2	335259	5	NULL	NULL	0	NULL	statement 1		failure of	leads to					p50		defect in generation of			NULL	T2 cells	0	NULL	NULL	NULL	gw60_jbiolchem_275_7_5238_s_231	10671572	Overall, these data suggest that the defect in p50 generation in T2 cells is due to a failure of proteasome-mediated cleavage of p105.	transcription
55793	1	335259	7	NULL	NULL	0	NULL	proteasome			mediates					p105		cleavage of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_7_5238_s_231	10671572	Overall, these data suggest that the defect in p50 generation in T2 cells is due to a failure of proteasome-mediated cleavage of p105.	transcription
55794	2	335259	7	NULL	NULL	0	NULL	p50		defect in generation of	is due to					statement 1		failure of			NULL	T2 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_7_5238_s_231	10671572	Overall, these data suggest that the defect in p50 generation in T2 cells is due to a failure of proteasome-mediated cleavage of p105.	transcription
54705	1	335261	5	NULL	NULL	0	NULL	p105			is a synonym of					NF-kappaB1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31244_s_5	8537390	Here, we report a  novel mechanism of NF-kappaB regulation mediated by p105 (NF-kappaB1)  precursor of p50 directly at the nuclear level.	transcription
54706	2	335261	5	NULL	NULL	0	NULL	p105			is a precursor of					p50					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31244_s_5	8537390	Here, we report a  novel mechanism of NF-kappaB regulation mediated by p105 (NF-kappaB1)  precursor of p50 directly at the nuclear level.	transcription
54707	3	335261	5	NULL	NULL	0	NULL	NF-kappaB		regulation of	is mediated by		directly			p105					NULL	nuclear level	0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31244_s_5	8537390	Here, we report a  novel mechanism of NF-kappaB regulation mediated by p105 (NF-kappaB1)  precursor of p50 directly at the nuclear level.	transcription
55795	1	335261	7	NULL	NULL	0	NULL	p105			mediates					NF-kappaB 		regulation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31244_s_5	8537390	Here, we report a  novel mechanism of NF-kappaB regulation mediated by p105 (NF-kappaB1)  precursor of p50 directly at the nuclear level.	transcription
55806	2	335261	7	NULL	NULL	0	NULL	p105			is a precursor of					p50					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31244_s_5	8537390	Here, we report a  novel mechanism of NF-kappaB regulation mediated by p105 (NF-kappaB1)  precursor of p50 directly at the nuclear level.	transcription
55807	3	335261	7	NULL	NULL	0	NULL	p105			is					NF-kappaB1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31244_s_5	8537390	Here, we report a  novel mechanism of NF-kappaB regulation mediated by p105 (NF-kappaB1)  precursor of p50 directly at the nuclear level.	transcription
55808	4	335261	7	NULL	NULL	0	NULL	statement 1			occurs at					nuclear level					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31244_s_5	8537390	Here, we report a  novel mechanism of NF-kappaB regulation mediated by p105 (NF-kappaB1)  precursor of p50 directly at the nuclear level.	transcription
54708	1	335262	5	NULL	NULL	0	NULL	mitomycin C			activates					NF-kappaB					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31244_s_157	8537390	Interestingly, concomitantly with  NF-kappaB activation by mitomycin C, p105 was processed to p50 in the  nucleus but not in the cytoplasm.	transcription
54709	2	335262	5	NULL	NULL	0	NULL	p105			is processed to					p50					NULL	nucleus	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31244_s_157	8537390	Interestingly, concomitantly with  NF-kappaB activation by mitomycin C, p105 was processed to p50 in the  nucleus but not in the cytoplasm.	transcription
54710	3	335262	5	NULL	NULL	0	NULL	statement 1			is concomitant to					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31244_s_157	8537390	Interestingly, concomitantly with  NF-kappaB activation by mitomycin C, p105 was processed to p50 in the  nucleus but not in the cytoplasm.	transcription
55809	1	335262	7	NULL	NULL	0	NULL	mitomycin C			activate					NF-kappaB					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31244_s_157	8537390	Interestingly, concomitantly with  NF-kappaB activation by mitomycin C, p105 was processed to p50 in the  nucleus but not in the cytoplasm.	transcription
55810	2	335262	7	NULL	NULL	0	NULL	p105			processed to					p50					NULL	nucleus	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31244_s_157	8537390	Interestingly, concomitantly with  NF-kappaB activation by mitomycin C, p105 was processed to p50 in the  nucleus but not in the cytoplasm.	transcription
55811	3	335262	7	NULL	NULL	0	NULL	statement 2			occurs upon					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31244_s_157	8537390	Interestingly, concomitantly with  NF-kappaB activation by mitomycin C, p105 was processed to p50 in the  nucleus but not in the cytoplasm.	transcription
55812	4	335262	7	NULL	NULL	0	NULL	p105			not processed to					p50					NULL	cytoplasm	0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31244_s_157	8537390	Interestingly, concomitantly with  NF-kappaB activation by mitomycin C, p105 was processed to p50 in the  nucleus but not in the cytoplasm.	transcription
54711	1	335263	5	NULL	NULL	0	NULL	C2-ceramide			induce					p105		processing of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_25_15494_s_43	9624136	However, C2-ceramide can induce p105 processing, with NFkappaB complexes predominantly comprising p50 homodimers.	transcription
54712	2	335263	5	NULL	NULL	0	NULL	NFkappaB complexes			compromises		predominantly			p50 homodimers					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_25_15494_s_43	9624136	However, C2-ceramide can induce p105 processing, with NFkappaB complexes predominantly comprising p50 homodimers.	transcription
55837	1	335263	7	NULL	NULL	0	NULL	C2-ceramide			induce					p105		processing of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_25_15494_s_43	9624136	However, C2-ceramide can induce p105 processing, with NFkappaB complexes predominantly comprising p50 homodimers.	transcription
55838	2	335263	7	NULL	NULL	0	NULL	NFkappaB complexes			comprise		predominantly			p50 homodimers					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_25_15494_s_43	9624136	However, C2-ceramide can induce p105 processing, with NFkappaB complexes predominantly comprising p50 homodimers.	transcription
54713	1	335264	5	NULL	NULL	0	NULL	NFkappaB1 gene			is autoregulated by		positively			NF-kappaB					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_3_1409_s_27	9430676	Since the NFkappaB1 gene is positively autoregulated by NF-kappaB, the increase in p50 could result in the presence of more p105 ( 31).	transcription
54714	2	335264	5	NULL	NULL	0	NULL	p50		increase in	results in					p105		presence of more			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_3_1409_s_27	9430676	Since the NFkappaB1 gene is positively autoregulated by NF-kappaB, the increase in p50 could result in the presence of more p105 ( 31).	transcription
54715	3	335264	5	NULL	NULL	0	NULL	statement 1			leads to					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_3_1409_s_27	9430676	Since the NFkappaB1 gene is positively autoregulated by NF-kappaB, the increase in p50 could result in the presence of more p105 ( 31).	transcription
55839	1	335264	7	NULL	NULL	0	NULL	NF-kappaB			autoregulates		positively			NFkappaB1 gene					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_3_1409_s_27	9430676	Since the NFkappaB1 gene is positively autoregulated by NF-kappaB, the increase in p50 could result in the presence of more p105 ( 31).	transcription
55840	2	335264	7	NULL	NULL	0	NULL	p50		increase in	in the presence of					p105					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_3_1409_s_27	9430676	Since the NFkappaB1 gene is positively autoregulated by NF-kappaB, the increase in p50 could result in the presence of more p105 ( 31).	transcription
55841	3	335264	7	NULL	NULL	0	NULL	statement 2			follows					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_3_1409_s_27	9430676	Since the NFkappaB1 gene is positively autoregulated by NF-kappaB, the increase in p50 could result in the presence of more p105 ( 31).	transcription
54716	1	335265	5	NULL	NULL	0	NULL	p105			is processed to					p50					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_3_1409_s_150	9430676	The  cim5-1 strain also inhibited processing of p105 to p50 at the non-permissive temperature (Fig.  2,  lane 5).	transcription
54717	2	335265	5	NULL	NULL	0	NULL	cim5-1 strain			inhibits					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_3_1409_s_150	9430676	The  cim5-1 strain also inhibited processing of p105 to p50 at the non-permissive temperature (Fig.  2,  lane 5).	transcription
55842	1	335265	7	NULL	NULL	0	NULL	p105			processed to					p50					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_3_1409_s_150	9430676	The  cim5-1 strain also inhibited processing of p105 to p50 at the non-permissive temperature (Fig.  2,  lane 5).	transcription
55843	2	335265	7	NULL	NULL	0	NULL	cim5-1 strain			inhibits					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_3_1409_s_150	9430676	The  cim5-1 strain also inhibited processing of p105 to p50 at the non-permissive temperature (Fig.  2,  lane 5).	transcription
55844	3	335265	7	NULL	NULL	0	NULL	statement 2			occurs at					non-permissive temperature 					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_3_1409_s_150	9430676	The  cim5-1 strain also inhibited processing of p105 to p50 at the non-permissive temperature (Fig.  2,  lane 5).	transcription
54718	1	335266	5	NULL	NULL	0	NULL	NF-kappaB1			is a precursor of			p105		NF-kappaB1			p50		NULL		0	NULL	NULL	NULL	abs-batch0680-0699_mol-cell-biol_23_1_12482991_s_2	12482991	NF-kappaB1 p105 functions both as a precursor of NF-kappaB1 p50 and as  a cytoplasmic inhibitor of NF-kappaB.	transcription
54719	2	335266	5	NULL	NULL	0	NULL	NF-kappaB1			is an inhibitor of			p105		NF-kappaB					NULL	cytoplasm	0	NULL	NULL	NULL	abs-batch0680-0699_mol-cell-biol_23_1_12482991_s_2	12482991	NF-kappaB1 p105 functions both as a precursor of NF-kappaB1 p50 and as  a cytoplasmic inhibitor of NF-kappaB.	transcription
55845	1	335266	7	NULL	NULL	0	NULL	NF-kappaB1 p105			functions as a					NF-kappaB1 p50		precursor of			NULL		0	NULL	NULL	NULL	abs-batch0680-0699_mol-cell-biol_23_1_12482991_s_2	12482991	NF-kappaB1 p105 functions both as a precursor of NF-kappaB1 p50 and as  a cytoplasmic inhibitor of NF-kappaB.	transcription
55846	2	335266	7	NULL	NULL	0	NULL	NF-kappaB1 p105 			functions as a					NF-kappaB		 cytoplasmic inhibitor of			NULL		0	NULL	NULL	NULL	abs-batch0680-0699_mol-cell-biol_23_1_12482991_s_2	12482991	NF-kappaB1 p105 functions both as a precursor of NF-kappaB1 p50 and as  a cytoplasmic inhibitor of NF-kappaB.	transcription
54720	1	335267	5	NULL	NULL	0	NULL	p50			corresponds to					p105			N terminus		NULL		0	NULL	NULL	NULL	abs-batch0720-0739_cell_92_6_9529257_s_3	9529257	p50 corresponds to the N terminus of p105 and with p65 (RelA)  forms the prototypical NF-kappaB transcription factor complex.	transcription
54721	2	335267	5	NULL	NULL	0	NULL	p65			is a synonym of					RelA					NULL		0	NULL	NULL	NULL	abs-batch0720-0739_cell_92_6_9529257_s_3	9529257	p50 corresponds to the N terminus of p105 and with p65 (RelA)  forms the prototypical NF-kappaB transcription factor complex.	transcription
54722	3	335267	5	NULL	NULL	0	NULL	p50			is a part of					NF-kappaB complex		prototypical			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_cell_92_6_9529257_s_3	9529257	p50 corresponds to the N terminus of p105 and with p65 (RelA)  forms the prototypical NF-kappaB transcription factor complex.	transcription
54723	4	335267	5	NULL	NULL	0	NULL	p65			is a part of					NF-kappaB complex		prototypical			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_cell_92_6_9529257_s_3	9529257	p50 corresponds to the N terminus of p105 and with p65 (RelA)  forms the prototypical NF-kappaB transcription factor complex.	transcription
54724	5	335267	5	NULL	NULL	0	NULL	statement 3			occurs along with					statement 4					NULL		0	NULL	NULL	NULL	abs-batch0720-0739_cell_92_6_9529257_s_3	9529257	p50 corresponds to the N terminus of p105 and with p65 (RelA)  forms the prototypical NF-kappaB transcription factor complex.	transcription
54725	6	335267	5	NULL	NULL	0	NULL	NF-kappaB			is a type of					transcription factor					NULL		0	NULL	NULL	NULL	abs-batch0720-0739_cell_92_6_9529257_s_3	9529257	p50 corresponds to the N terminus of p105 and with p65 (RelA)  forms the prototypical NF-kappaB transcription factor complex.	transcription
55847	1	335267	7	NULL	NULL	0	NULL	p50			corresponds to					p105			N terminus		NULL		0	NULL	NULL	NULL	abs-batch0720-0739_cell_92_6_9529257_s_3	9529257	p50 corresponds to the N terminus of p105 and with p65 (RelA)  forms the prototypical NF-kappaB transcription factor complex.	transcription
55848	2	335267	7	NULL	NULL	0	NULL	p50			associate with					p65					NULL		0	NULL	NULL	NULL	abs-batch0720-0739_cell_92_6_9529257_s_3	9529257	p50 corresponds to the N terminus of p105 and with p65 (RelA)  forms the prototypical NF-kappaB transcription factor complex.	transcription
55849	3	335267	7	NULL	NULL	0	NULL	statement 2			forms					prototypical NF-kappaB transcription factor complex					NULL		0	NULL	NULL	NULL	abs-batch0720-0739_cell_92_6_9529257_s_3	9529257	p50 corresponds to the N terminus of p105 and with p65 (RelA)  forms the prototypical NF-kappaB transcription factor complex.	transcription
55850	4	335267	7	NULL	NULL	0	NULL	p65			is					RelA					NULL		0	NULL	NULL	NULL	abs-batch0720-0739_cell_92_6_9529257_s_3	9529257	p50 corresponds to the N terminus of p105 and with p65 (RelA)  forms the prototypical NF-kappaB transcription factor complex.	transcription
54726	1	335268	5	NULL	NULL	0	NULL	GSK-3beta			phosphorylates					p105					NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_261	16192643	In addition, GSK-3beta phosphorylates the p105 precursor of the p50 member of the NF-kappaB dimer; this has the dual effect of slowing constitutive processing to p50 and accelerating the degradation of p50 on stimulation with TNF-alpha.	transcription
54727	2	335268	5	NULL	NULL	0	NULL	p105			is a precursor of					p50					NULL		NULL	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_261	16192643	In addition, GSK-3beta phosphorylates the p105 precursor of the p50 member of the NF-kappaB dimer; this has the dual effect of slowing constitutive processing to p50 and accelerating the degradation of p50 on stimulation with TNF-alpha.	transcription
54728	3	335268	5	NULL	NULL	0	NULL	p50			is a member of					NF-kappaB dimer					NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_261	16192643	In addition, GSK-3beta phosphorylates the p105 precursor of the p50 member of the NF-kappaB dimer; this has the dual effect of slowing constitutive processing to p50 and accelerating the degradation of p50 on stimulation with TNF-alpha.	transcription
54729	4	335268	5	NULL	NULL	0	NULL	p105			is processed to		constitutive			p50					NULL		NULL	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_261	16192643	In addition, GSK-3beta phosphorylates the p105 precursor of the p50 member of the NF-kappaB dimer; this has the dual effect of slowing constitutive processing to p50 and accelerating the degradation of p50 on stimulation with TNF-alpha.	transcription
54730	5	335268	5	NULL	NULL	0	NULL	statement 1			slows					statement 4					NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_261	16192643	In addition, GSK-3beta phosphorylates the p105 precursor of the p50 member of the NF-kappaB dimer; this has the dual effect of slowing constitutive processing to p50 and accelerating the degradation of p50 on stimulation with TNF-alpha.	transcription
54731	6	335268	5	NULL	NULL	0	NULL	statement 1			accelerates					p50		degradation of			NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_261	16192643	In addition, GSK-3beta phosphorylates the p105 precursor of the p50 member of the NF-kappaB dimer; this has the dual effect of slowing constitutive processing to p50 and accelerating the degradation of p50 on stimulation with TNF-alpha.	transcription
54732	7	335268	5	NULL	NULL	0	NULL	TNF-alpha		stimulation	leads to					statement 6					NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_261	16192643	In addition, GSK-3beta phosphorylates the p105 precursor of the p50 member of the NF-kappaB dimer; this has the dual effect of slowing constitutive processing to p50 and accelerating the degradation of p50 on stimulation with TNF-alpha.	transcription
55851	1	335268	7	NULL	NULL	0	NULL	 GSK-3beta			phosphorylates					NF-kappaB dimer		p105 precursor of;; p50 member of 			NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_261	16192643	In addition, GSK-3beta phosphorylates the p105 precursor of the p50 member of the NF-kappaB dimer; this has the dual effect of slowing constitutive processing to p50 and accelerating the degradation of p50 on stimulation with TNF-alpha.	transcription
55852	2	335268	7	NULL	NULL	0	NULL	statement 1			slows					p50		 constitutive processing to 			NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_261	16192643	In addition, GSK-3beta phosphorylates the p105 precursor of the p50 member of the NF-kappaB dimer; this has the dual effect of slowing constitutive processing to p50 and accelerating the degradation of p50 on stimulation with TNF-alpha.	transcription
55853	3	335268	7	NULL	NULL	0	NULL	TNF-alpha		stimulation with 	degrades					p50					NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_261	16192643	In addition, GSK-3beta phosphorylates the p105 precursor of the p50 member of the NF-kappaB dimer; this has the dual effect of slowing constitutive processing to p50 and accelerating the degradation of p50 on stimulation with TNF-alpha.	transcription
55854	4	335268	7	NULL	NULL	0	NULL	statement 1			accelerates					statement 3					NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_261	16192643	In addition, GSK-3beta phosphorylates the p105 precursor of the p50 member of the NF-kappaB dimer; this has the dual effect of slowing constitutive processing to p50 and accelerating the degradation of p50 on stimulation with TNF-alpha.	transcription
54733	1	335269	5	NULL	NULL	0	NULL	p105			bind					NF-kappaB protein					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_1_556_s_131	12399470	The fact that p105 binds to all NF-kappaB proteins and IkappaBgamma binds only to p50 dimers (any NF-kappaB dimer that contains at least one p50 subunit) suggests that the required p50 subunit in IkappaBgamma.	transcription
54734	2	335269	5	NULL	NULL	0	NULL	IkappaBgamma			bind					p50 dimers					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_1_556_s_131	12399470	The fact that p105 binds to all NF-kappaB proteins and IkappaBgamma binds only to p50 dimers (any NF-kappaB dimer that contains at least one p50 subunit) suggests that the required p50 subunit in IkappaBgamma.	transcription
55855	1	335269	7	NULL	NULL	0	NULL	 p105			bind					NF-kappaB proteins					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_1_556_s_131	12399470	The fact that p105 binds to all NF-kappaB proteins and IkappaBgamma binds only to p50 dimers (any NF-kappaB dimer that contains at least one p50 subunit) suggests that the required p50 subunit in IkappaBgamma.	transcription
55856	2	335269	7	NULL	NULL	0	NULL	 IkappaBgamma			bind		only			p50 dimer					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_1_556_s_131	12399470	The fact that p105 binds to all NF-kappaB proteins and IkappaBgamma binds only to p50 dimers (any NF-kappaB dimer that contains at least one p50 subunit) suggests that the required p50 subunit in IkappaBgamma.	transcription
55857	3	335269	7	NULL	NULL	0	NULL	statement 2			requires					 IkappaBgamma			p50 subunit		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_1_556_s_131	12399470	The fact that p105 binds to all NF-kappaB proteins and IkappaBgamma binds only to p50 dimers (any NF-kappaB dimer that contains at least one p50 subunit) suggests that the required p50 subunit in IkappaBgamma.	transcription
54735	1	335270	5	NULL	NULL	0	NULL	BCL-3			acts as					chaperone					NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_252	10970863	BCL-3 could act as a chaperone binding the p50 - p105 complex and promoting its disassembly while preserving the proper conformation in p50 for dimerization with other disassembled p50 monomers.	transcription
54736	2	335270	5	NULL	NULL	0	NULL	BCL-3			bind					p50 - p105 complex					NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_252	10970863	BCL-3 could act as a chaperone binding the p50 - p105 complex and promoting its disassembly while preserving the proper conformation in p50 for dimerization with other disassembled p50 monomers.	transcription
54737	3	335270	5	NULL	NULL	0	NULL	BCL-3			promotes					p50 - p105 complex		disassembly of			NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_252	10970863	BCL-3 could act as a chaperone binding the p50 - p105 complex and promoting its disassembly while preserving the proper conformation in p50 for dimerization with other disassembled p50 monomers.	transcription
54738	4	335270	5	NULL	NULL	0	NULL	statement 3			preserves					p50		proper conformation of			NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_252	10970863	BCL-3 could act as a chaperone binding the p50 - p105 complex and promoting its disassembly while preserving the proper conformation in p50 for dimerization with other disassembled p50 monomers.	transcription
54739	5	335270	5	NULL	NULL	0	NULL	p50			dimerize with					p50 monomers		disassembled			NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_252	10970863	BCL-3 could act as a chaperone binding the p50 - p105 complex and promoting its disassembly while preserving the proper conformation in p50 for dimerization with other disassembled p50 monomers.	transcription
54740	6	335270	5	NULL	NULL	0	NULL	statement 4			leads to					statement 5					NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_252	10970863	BCL-3 could act as a chaperone binding the p50 - p105 complex and promoting its disassembly while preserving the proper conformation in p50 for dimerization with other disassembled p50 monomers.	transcription
55858	1	335270	7	NULL	NULL	0	NULL	BCL-3			bind					p50 - p105 complex 					NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_252	10970863	BCL-3 could act as a chaperone binding the p50 - p105 complex and promoting its disassembly while preserving the proper conformation in p50 for dimerization with other disassembled p50 monomers.	transcription
55859	2	335270	7	NULL	NULL	0	NULL	BCL-3			act as a 					chaperone					NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_252	10970863	BCL-3 could act as a chaperone binding the p50 - p105 complex and promoting its disassembly while preserving the proper conformation in p50 for dimerization with other disassembled p50 monomers.	transcription
55860	3	335270	7	NULL	NULL	0	NULL	statement 1			promote					p50 - p105 complex		disassembly of			NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_252	10970863	BCL-3 could act as a chaperone binding the p50 - p105 complex and promoting its disassembly while preserving the proper conformation in p50 for dimerization with other disassembled p50 monomers.	transcription
55861	4	335270	7	NULL	NULL	0	NULL	BCL-3			preserve					p50		proper conformation of			NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_252	10970863	BCL-3 could act as a chaperone binding the p50 - p105 complex and promoting its disassembly while preserving the proper conformation in p50 for dimerization with other disassembled p50 monomers.	transcription
55862	5	335270	7	NULL	NULL	0	NULL	p50 			dimerize with					p50 monomers		disassembled			NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_252	10970863	BCL-3 could act as a chaperone binding the p50 - p105 complex and promoting its disassembly while preserving the proper conformation in p50 for dimerization with other disassembled p50 monomers.	transcription
55863	6	335270	7	NULL	NULL	0	NULL	statement 4			required for					statement 5					NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_252	10970863	BCL-3 could act as a chaperone binding the p50 - p105 complex and promoting its disassembly while preserving the proper conformation in p50 for dimerization with other disassembled p50 monomers.	transcription
54741	1	335271	5	NULL	NULL	0	NULL	p50			inhibits					p105		processing of			NULL	in vivo	0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_177	11350967	p50 Inhibits Processing of p105 in Vivo, and Inhibition Is Dependent on the Presence of the Ankyrin Repeat-containing Domain-- To test the effect of the ankyrin repeat domain and anchored p50 subunits on processing of p105  in vivo, we overexpressed p50- XbaI in cells that do not express the NF-kappaB cascade proteins.	transcription
54742	2	335271	5	NULL	NULL	0	NULL	statement 1			is dependent on							presence of	ankyrin repeat-containing domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_177	11350967	p50 Inhibits Processing of p105 in Vivo, and Inhibition Is Dependent on the Presence of the Ankyrin Repeat-containing Domain-- To test the effect of the ankyrin repeat domain and anchored p50 subunits on processing of p105  in vivo, we overexpressed p50- XbaI in cells that do not express the NF-kappaB cascade proteins.	transcription
55864	1	335271	7	NULL	NULL	0	NULL	p50			inhibits					p105		processing of			NULL	in vivo	0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_177	11350967	p50 Inhibits Processing of p105 in Vivo, and Inhibition Is Dependent on the Presence of the Ankyrin Repeat-containing Domain-- To test the effect of the ankyrin repeat domain and anchored p50 subunits on processing of p105  in vivo, we overexpressed p50- XbaI in cells that do not express the NF-kappaB cascade proteins.	transcription
55865	2	335271	7	NULL	NULL	0	NULL	statement 1			depends on							presence of	Ankyrin Repeat-containing Domain-		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_177	11350967	p50 Inhibits Processing of p105 in Vivo, and Inhibition Is Dependent on the Presence of the Ankyrin Repeat-containing Domain-- To test the effect of the ankyrin repeat domain and anchored p50 subunits on processing of p105  in vivo, we overexpressed p50- XbaI in cells that do not express the NF-kappaB cascade proteins.	transcription
54743	1	335272	5	NULL	NULL	0	NULL	BCL3			increases					p50 homodimers		quantity of			NULL	nucleus	0	NULL	NULL	NULL	gw60_jbiolchem_272_52_33132_s_290	9407099	Recently, it has been shown that BCL3 can increase the quantity of nuclear p50 homodimers by inducing a redistribution of the subunits of cytoplasmic heterodimers containing p50 and its precursor p105 to yield p50 homodimers that translocate to the nucleus; this occurs without an effect on processing of p105 ( 54).	transcription
54744	3	335272	5	NULL	NULL	0	NULL	BCL3			redistributes					statement 2					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_52_33132_s_290	9407099	Recently, it has been shown that BCL3 can increase the quantity of nuclear p50 homodimers by inducing a redistribution of the subunits of cytoplasmic heterodimers containing p50 and its precursor p105 to yield p50 homodimers that translocate to the nucleus; this occurs without an effect on processing of p105 ( 54).	transcription
54745	4	335272	5	NULL	NULL	0	NULL	statement 3			leads to					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_52_33132_s_290	9407099	Recently, it has been shown that BCL3 can increase the quantity of nuclear p50 homodimers by inducing a redistribution of the subunits of cytoplasmic heterodimers containing p50 and its precursor p105 to yield p50 homodimers that translocate to the nucleus; this occurs without an effect on processing of p105 ( 54).	transcription
54746	2	335272	5	NULL	NULL	0	NULL	p105 precursor			bind					p50					NULL	cytoplasm	0	NULL	NULL	NULL	gw60_jbiolchem_272_52_33132_s_290	9407099	Recently, it has been shown that BCL3 can increase the quantity of nuclear p50 homodimers by inducing a redistribution of the subunits of cytoplasmic heterodimers containing p50 and its precursor p105 to yield p50 homodimers that translocate to the nucleus; this occurs without an effect on processing of p105 ( 54).	transcription
54747	5	335272	5	NULL	NULL	0	NULL	statement 3			yields					p50 homodimers					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_52_33132_s_290	9407099	Recently, it has been shown that BCL3 can increase the quantity of nuclear p50 homodimers by inducing a redistribution of the subunits of cytoplasmic heterodimers containing p50 and its precursor p105 to yield p50 homodimers that translocate to the nucleus; this occurs without an effect on processing of p105 ( 54).	transcription
54748	6	335272	5	NULL	NULL	0	NULL	p50 homodimers			translocates to					nucleus					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_52_33132_s_290	9407099	Recently, it has been shown that BCL3 can increase the quantity of nuclear p50 homodimers by inducing a redistribution of the subunits of cytoplasmic heterodimers containing p50 and its precursor p105 to yield p50 homodimers that translocate to the nucleus; this occurs without an effect on processing of p105 ( 54).	transcription
54749	7	335272	5	NULL	NULL	0	NULL	statement 1			does not effect					p105		processing of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_52_33132_s_290	9407099	Recently, it has been shown that BCL3 can increase the quantity of nuclear p50 homodimers by inducing a redistribution of the subunits of cytoplasmic heterodimers containing p50 and its precursor p105 to yield p50 homodimers that translocate to the nucleus; this occurs without an effect on processing of p105 ( 54).	transcription
55866	1	335272	7	NULL	NULL	0	NULL	BCL3			increase					 p50 homodimers		quantity of;; nuclear			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_52_33132_s_290	9407099	Recently, it has been shown that BCL3 can increase the quantity of nuclear p50 homodimers by inducing a redistribution of the subunits of cytoplasmic heterodimers containing p50 and its precursor p105 to yield p50 homodimers that translocate to the nucleus; this occurs without an effect on processing of p105 ( 54).	transcription
55867	2	335272	7	NULL	NULL	0	NULL	p50			heterodimerize with					p105					NULL	cytoplasm	0	NULL	NULL	NULL	gw60_jbiolchem_272_52_33132_s_290	9407099	Recently, it has been shown that BCL3 can increase the quantity of nuclear p50 homodimers by inducing a redistribution of the subunits of cytoplasmic heterodimers containing p50 and its precursor p105 to yield p50 homodimers that translocate to the nucleus; this occurs without an effect on processing of p105 ( 54).	transcription
55868	3	335272	7	NULL	NULL	0	NULL	BCL3			induce					statement 2		redistribution of	subunits 		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_52_33132_s_290	9407099	Recently, it has been shown that BCL3 can increase the quantity of nuclear p50 homodimers by inducing a redistribution of the subunits of cytoplasmic heterodimers containing p50 and its precursor p105 to yield p50 homodimers that translocate to the nucleus; this occurs without an effect on processing of p105 ( 54).	transcription
55869	4	335272	7	NULL	NULL	0	NULL	statement 3			yield					p50 homodimers					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_52_33132_s_290	9407099	Recently, it has been shown that BCL3 can increase the quantity of nuclear p50 homodimers by inducing a redistribution of the subunits of cytoplasmic heterodimers containing p50 and its precursor p105 to yield p50 homodimers that translocate to the nucleus; this occurs without an effect on processing of p105 ( 54).	transcription
55870	5	335272	7	NULL	NULL	0	NULL	p50 homodimers			translocate to					nucleus					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_52_33132_s_290	9407099	Recently, it has been shown that BCL3 can increase the quantity of nuclear p50 homodimers by inducing a redistribution of the subunits of cytoplasmic heterodimers containing p50 and its precursor p105 to yield p50 homodimers that translocate to the nucleus; this occurs without an effect on processing of p105 ( 54).	transcription
55871	6	335272	7	NULL	NULL	0	NULL	statement 5			does not effect					p105		processing of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_52_33132_s_290	9407099	Recently, it has been shown that BCL3 can increase the quantity of nuclear p50 homodimers by inducing a redistribution of the subunits of cytoplasmic heterodimers containing p50 and its precursor p105 to yield p50 homodimers that translocate to the nucleus; this occurs without an effect on processing of p105 ( 54).	transcription
55872	7	335272	7	NULL	NULL	0	NULL	p105			is a precursor of					p50					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_52_33132_s_290	9407099	Recently, it has been shown that BCL3 can increase the quantity of nuclear p50 homodimers by inducing a redistribution of the subunits of cytoplasmic heterodimers containing p50 and its precursor p105 to yield p50 homodimers that translocate to the nucleus; this occurs without an effect on processing of p105 ( 54).	transcription
54750	1	335273	5	NULL	NULL	0	NULL				resides in			serines		p105			PEST domain		NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_12_5235_s_18	15169888	However, following cellular stimulation with ligands, such as TNF-alpha, two serines in the p105 PEST domain are rapidly phosphorylated by the IkappaB kinase (IKK) complex, triggering complete p105 degradation with little effect on processing to p50 ( ,  ,  ).	transcription
54751	2	335273	5	NULL	NULL	0	NULL	IKK			phosphorylates		rapidly			statement 1					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_12_5235_s_18	15169888	However, following cellular stimulation with ligands, such as TNF-alpha, two serines in the p105 PEST domain are rapidly phosphorylated by the IkappaB kinase (IKK) complex, triggering complete p105 degradation with little effect on processing to p50 ( ,  ,  ).	transcription
54753	3	335273	5	NULL	NULL	0	NULL	IKK			is					IkappaB kinase complex					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_12_5235_s_18	15169888	However, following cellular stimulation with ligands, such as TNF-alpha, two serines in the p105 PEST domain are rapidly phosphorylated by the IkappaB kinase (IKK) complex, triggering complete p105 degradation with little effect on processing to p50 ( ,  ,  ).	transcription
54754	4	335273	5	NULL	NULL	0	NULL	TNF-alpha			is a type of					ligand					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_12_5235_s_18	15169888	However, following cellular stimulation with ligands, such as TNF-alpha, two serines in the p105 PEST domain are rapidly phosphorylated by the IkappaB kinase (IKK) complex, triggering complete p105 degradation with little effect on processing to p50 ( ,  ,  ).	transcription
54755	5	335273	5	NULL	NULL	0	NULL	TNF-alpha			stimulates					statement 2					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_12_5235_s_18	15169888	However, following cellular stimulation with ligands, such as TNF-alpha, two serines in the p105 PEST domain are rapidly phosphorylated by the IkappaB kinase (IKK) complex, triggering complete p105 degradation with little effect on processing to p50 ( ,  ,  ).	transcription
54756	6	335273	5	NULL	NULL	0	NULL	statement 2			triggers					p105		complete degradation of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_12_5235_s_18	15169888	However, following cellular stimulation with ligands, such as TNF-alpha, two serines in the p105 PEST domain are rapidly phosphorylated by the IkappaB kinase (IKK) complex, triggering complete p105 degradation with little effect on processing to p50 ( ,  ,  ).	transcription
54757	7	335273	5	NULL	NULL	0	NULL	p105			is processed to					p50					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_12_5235_s_18	15169888	However, following cellular stimulation with ligands, such as TNF-alpha, two serines in the p105 PEST domain are rapidly phosphorylated by the IkappaB kinase (IKK) complex, triggering complete p105 degradation with little effect on processing to p50 ( ,  ,  ).	transcription
54758	8	335273	5	NULL	NULL	0	NULL	statement 6			does not effect					statement 7					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_12_5235_s_18	15169888	However, following cellular stimulation with ligands, such as TNF-alpha, two serines in the p105 PEST domain are rapidly phosphorylated by the IkappaB kinase (IKK) complex, triggering complete p105 degradation with little effect on processing to p50 ( ,  ,  ).	transcription
55873	1	335273	7	NULL	NULL	0	NULL	TNF-alpha			stimulate					cells					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_12_5235_s_18	15169888	However, following cellular stimulation with ligands, such as TNF-alpha, two serines in the p105 PEST domain are rapidly phosphorylated by the IkappaB kinase (IKK) complex, triggering complete p105 degradation with little effect on processing to p50 ( ,  ,  ).	transcription
55874	2	335273	7	NULL	NULL	0	NULL	IKK complex			phosphorylate		rapidly			p105			two serines in the PEST domain		NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_12_5235_s_18	15169888	However, following cellular stimulation with ligands, such as TNF-alpha, two serines in the p105 PEST domain are rapidly phosphorylated by the IkappaB kinase (IKK) complex, triggering complete p105 degradation with little effect on processing to p50 ( ,  ,  ).	transcription
55875	3	335273	7	NULL	NULL	0	NULL	statement 2			is followed by 					statement 1					NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_12_5235_s_18	15169888	However, following cellular stimulation with ligands, such as TNF-alpha, two serines in the p105 PEST domain are rapidly phosphorylated by the IkappaB kinase (IKK) complex, triggering complete p105 degradation with little effect on processing to p50 ( ,  ,  ).	transcription
55876	4	335273	7	NULL	NULL	0	NULL	statement 2			trigger					p105		complete degradation of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_12_5235_s_18	15169888	However, following cellular stimulation with ligands, such as TNF-alpha, two serines in the p105 PEST domain are rapidly phosphorylated by the IkappaB kinase (IKK) complex, triggering complete p105 degradation with little effect on processing to p50 ( ,  ,  ).	transcription
55877	5	335273	7	NULL	NULL	0	NULL	statement 2			effect on		little			p50		processing to			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_12_5235_s_18	15169888	However, following cellular stimulation with ligands, such as TNF-alpha, two serines in the p105 PEST domain are rapidly phosphorylated by the IkappaB kinase (IKK) complex, triggering complete p105 degradation with little effect on processing to p50 ( ,  ,  ).	transcription
55878	6	335273	7	NULL	NULL	0	NULL	IKK			is					IkappaB kinase 					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_12_5235_s_18	15169888	However, following cellular stimulation with ligands, such as TNF-alpha, two serines in the p105 PEST domain are rapidly phosphorylated by the IkappaB kinase (IKK) complex, triggering complete p105 degradation with little effect on processing to p50 ( ,  ,  ).	transcription
54759	1	335274	5	NULL	NULL	0	NULL	TPL-2			increase		may			Myc - p105		efficiency of;;processing of			NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_77	9950430	As Myc - p50 was generated at a similar rate in cells co-transfected with TPL-2 as in control cells, but from progressively decreasing amounts of Myc - p105 ( Fig. 6c), TPL-2 may increase the efficiency of Myc - p105 processing.	transcription
55879	1	335274	7	NULL	NULL	0	NULL	TPL-2 			increase		may			Myc - p105		efficiency of;; processing of			NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_77	9950430	As Myc - p50 was generated at a similar rate in cells co-transfected with TPL-2 as in control cells, but from progressively decreasing amounts of Myc - p105 ( Fig. 6c), TPL-2 may increase the efficiency of Myc - p105 processing.	transcription
55880	2	335274	7	NULL	NULL	0	NULL	statement 1			occurs upon					Myc - p105 		progressively decreasing amounts of			NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_77	9950430	As Myc - p50 was generated at a similar rate in cells co-transfected with TPL-2 as in control cells, but from progressively decreasing amounts of Myc - p105 ( Fig. 6c), TPL-2 may increase the efficiency of Myc - p105 processing.	transcription
54760	1	335275	5	NULL	NULL	0	NULL	MG132			is an inhibitor of		potent			proteasome 4					NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_83	9950430	Treatment with MG132, a potent inhibitor of the proteasome 4, blocked increased turnover of Myc - p105 ( Fig. 6f) and completely prevented Myc - p50 production (data not shown) in cells co-expressing TPL-2 and Myc - p105.	transcription
54761	2	335275	5	NULL	NULL	0	NULL	MG132		treatment	blocks					Myc - p105		increased turnover of			NULL	cells co-expressing TPL-2 and Myc - p105	NULL	NULL	NULL	NULL	gw60_nature_397_6717_363_s_83	9950430	Treatment with MG132, a potent inhibitor of the proteasome 4, blocked increased turnover of Myc - p105 ( Fig. 6f) and completely prevented Myc - p50 production (data not shown) in cells co-expressing TPL-2 and Myc - p105.	transcription
54762	3	335275	5	NULL	NULL	0	NULL	MG132		treatment	prevented		completely			Myc - p50		production of			NULL	cells co-expressing TPL-2 and Myc - p105	0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_83	9950430	Treatment with MG132, a potent inhibitor of the proteasome 4, blocked increased turnover of Myc - p105 ( Fig. 6f) and completely prevented Myc - p50 production (data not shown) in cells co-expressing TPL-2 and Myc - p105.	transcription
55881	1	335275	7	NULL	NULL	0	NULL	MG132			blocks					Myc - p105 		increased turnover of			NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_83	9950430	Treatment with MG132, a potent inhibitor of the proteasome 4, blocked increased turnover of Myc - p105 ( Fig. 6f) and completely prevented Myc - p50 production (data not shown) in cells co-expressing TPL-2 and Myc - p105.	transcription
55882	2	335275	7	NULL	NULL	0	NULL	MG132			is a type of					proteasome 4 inhibitor					NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_83	9950430	Treatment with MG132, a potent inhibitor of the proteasome 4, blocked increased turnover of Myc - p105 ( Fig. 6f) and completely prevented Myc - p50 production (data not shown) in cells co-expressing TPL-2 and Myc - p105.	transcription
55883	3	335275	7	NULL	NULL	0	NULL	MG132			prevents		completely			Myc - p50		production of			NULL	cells co-expressing TPL-2 and Myc - p105	NULL	NULL	NULL	NULL	gw60_nature_397_6717_363_s_83	9950430	Treatment with MG132, a potent inhibitor of the proteasome 4, blocked increased turnover of Myc - p105 ( Fig. 6f) and completely prevented Myc - p50 production (data not shown) in cells co-expressing TPL-2 and Myc - p105.	transcription
54778	1	335276	5	NULL	NULL	0	NULL	Myc - p105			is degraded by					proteasome					NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_84	9950430	Thus, the results of the metabolic labelling experiments (above) indicate that the predominant effect of TPL-2 expression is to increase the rate of Myc - p105 degradation by the proteasome while maintaining the overall rate of production of Myc - p50 from Myc - p105.	transcription
54779	2	335276	5	NULL	NULL	0	NULL	Myc - p50			is produced from					Myc - p105					NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_84	9950430	Thus, the results of the metabolic labelling experiments (above) indicate that the predominant effect of TPL-2 expression is to increase the rate of Myc - p105 degradation by the proteasome while maintaining the overall rate of production of Myc - p50 from Myc - p105.	transcription
54780	3	335276	5	NULL	NULL	0	NULL	TPL-2		expression of	increases					statement 1		rate of			NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_84	9950430	Thus, the results of the metabolic labelling experiments (above) indicate that the predominant effect of TPL-2 expression is to increase the rate of Myc - p105 degradation by the proteasome while maintaining the overall rate of production of Myc - p50 from Myc - p105.	transcription
54781	4	335276	5	NULL	NULL	0	NULL	TPL-2		expression of	maintains					statement 2		overall rate of			NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_84	9950430	Thus, the results of the metabolic labelling experiments (above) indicate that the predominant effect of TPL-2 expression is to increase the rate of Myc - p105 degradation by the proteasome while maintaining the overall rate of production of Myc - p50 from Myc - p105.	transcription
54782	5	335276	5	NULL	NULL	0	NULL	statement 3			occurs simultaneously with					statement 4					NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_84	9950430	Thus, the results of the metabolic labelling experiments (above) indicate that the predominant effect of TPL-2 expression is to increase the rate of Myc - p105 degradation by the proteasome while maintaining the overall rate of production of Myc - p50 from Myc - p105.	transcription
55884	1	335276	7	NULL	NULL	0	NULL	proteasome 			degrades					Myc - p105					NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_84	9950430	Thus, the results of the metabolic labelling experiments (above) indicate that the predominant effect of TPL-2 expression is to increase the rate of Myc - p105 degradation by the proteasome while maintaining the overall rate of production of Myc - p50 from Myc - p105.	transcription
55885	2	335276	7	NULL	NULL	0	NULL	TPL-2		expression of	increase					statement 1					NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_84	9950430	Thus, the results of the metabolic labelling experiments (above) indicate that the predominant effect of TPL-2 expression is to increase the rate of Myc - p105 degradation by the proteasome while maintaining the overall rate of production of Myc - p50 from Myc - p105.	transcription
55886	3	335276	7	NULL	NULL	0	NULL	Myc - p50			produced from					Myc - p105					NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_84	9950430	Thus, the results of the metabolic labelling experiments (above) indicate that the predominant effect of TPL-2 expression is to increase the rate of Myc - p105 degradation by the proteasome while maintaining the overall rate of production of Myc - p50 from Myc - p105.	transcription
55887	4	335276	7	NULL	NULL	0	NULL	TPL-2 		expression of	maintains					statement 3					NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_84	9950430	Thus, the results of the metabolic labelling experiments (above) indicate that the predominant effect of TPL-2 expression is to increase the rate of Myc - p105 degradation by the proteasome while maintaining the overall rate of production of Myc - p50 from Myc - p105.	transcription
54783	1	335277	5	NULL	NULL	0	NULL	Tpl2			forms a complex with		stable			p105					NULL		0	NULL	NULL	NULL	gw60_molcell_11_3_685_s_169	12667451	Interestingly, the coIP assays revealed that while Tpl2 formed a stable complex with p105 (  Figure 4C, top panel, lane 2) and p105 N (lane 6), it did not interact with p50 (lane 3) or p100 (lane 4).	transcription
54784	2	335277	5	NULL	NULL	0	NULL	Tpl2			forms a complex with		stable			p105 N					NULL		0	NULL	NULL	NULL	gw60_molcell_11_3_685_s_169	12667451	Interestingly, the coIP assays revealed that while Tpl2 formed a stable complex with p105 (  Figure 4C, top panel, lane 2) and p105 N (lane 6), it did not interact with p50 (lane 3) or p100 (lane 4).	transcription
54785	3	335277	5	NULL	NULL	0	NULL	Tpl2			does not interact with					p50					NULL		0	NULL	NULL	NULL	gw60_molcell_11_3_685_s_169	12667451	Interestingly, the coIP assays revealed that while Tpl2 formed a stable complex with p105 (  Figure 4C, top panel, lane 2) and p105 N (lane 6), it did not interact with p50 (lane 3) or p100 (lane 4).	transcription
54786	4	335277	5	NULL	NULL	0	NULL	Tpl2			does not interact with					p100					NULL		0	NULL	NULL	NULL	gw60_molcell_11_3_685_s_169	12667451	Interestingly, the coIP assays revealed that while Tpl2 formed a stable complex with p105 (  Figure 4C, top panel, lane 2) and p105 N (lane 6), it did not interact with p50 (lane 3) or p100 (lane 4).	transcription
54787	5	335277	5	NULL	NULL	0	NULL	statement 3			is an alternative to					statement 4					NULL		0	NULL	NULL	NULL	gw60_molcell_11_3_685_s_169	12667451	Interestingly, the coIP assays revealed that while Tpl2 formed a stable complex with p105 (  Figure 4C, top panel, lane 2) and p105 N (lane 6), it did not interact with p50 (lane 3) or p100 (lane 4).	transcription
55888	1	335277	7	NULL	NULL	0	NULL	Tpl2			forms stable complex with					p105					NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_3_685_s_169	12667451	Interestingly, the coIP assays revealed that while Tpl2 formed a stable complex with p105 (  Figure 4C, top panel, lane 2) and p105 N (lane 6), it did not interact with p50 (lane 3) or p100 (lane 4).	transcription
55889	2	335277	7	NULL	NULL	0	NULL	Tpl2			forms stable complex with					p105 N					NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_3_685_s_169	12667451	Interestingly, the coIP assays revealed that while Tpl2 formed a stable complex with p105 (  Figure 4C, top panel, lane 2) and p105 N (lane 6), it did not interact with p50 (lane 3) or p100 (lane 4).	transcription
55890	3	335277	7	NULL	NULL	0	NULL	Tpl2			does not interact with					p50					NULL		0	NULL	NULL	NULL	gw60_molcell_11_3_685_s_169	12667451	Interestingly, the coIP assays revealed that while Tpl2 formed a stable complex with p105 (  Figure 4C, top panel, lane 2) and p105 N (lane 6), it did not interact with p50 (lane 3) or p100 (lane 4).	transcription
55891	4	335277	7	NULL	NULL	0	NULL	Tpl2			does not interact with					p100					NULL		0	NULL	NULL	NULL	gw60_molcell_11_3_685_s_169	12667451	Interestingly, the coIP assays revealed that while Tpl2 formed a stable complex with p105 (  Figure 4C, top panel, lane 2) and p105 N (lane 6), it did not interact with p50 (lane 3) or p100 (lane 4).	transcription
54788	1	335278	5	NULL	NULL	0	NULL	p105			is processed to					p50					NULL	nucleus	0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31244_s_7	8537390	In concomitance with NF-kappaB activation,  mitomycin C induced the processing of p105 to p50 in the nucleus, while  it did not affect the steady-state protein levels of IkappaBalpha  and  p105 in the cytoplasm.	transcription
54789	2	335278	5	NULL	NULL	0	NULL	mitomycin C			induce					statement 1					NULL	nucleus	0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31244_s_7	8537390	In concomitance with NF-kappaB activation,  mitomycin C induced the processing of p105 to p50 in the nucleus, while  it did not affect the steady-state protein levels of IkappaBalpha  and  p105 in the cytoplasm.	transcription
54790	3	335278	5	NULL	NULL	0	NULL	NF-kappaB		activation of	is concomitant to					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31244_s_7	8537390	In concomitance with NF-kappaB activation,  mitomycin C induced the processing of p105 to p50 in the nucleus, while  it did not affect the steady-state protein levels of IkappaBalpha  and  p105 in the cytoplasm.	transcription
54791	4	335278	5	NULL	NULL	0	NULL	mitomycin C			does not affect					IkappaBalpha		protein levels of			NULL	cytoplasm	0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31244_s_7	8537390	In concomitance with NF-kappaB activation,  mitomycin C induced the processing of p105 to p50 in the nucleus, while  it did not affect the steady-state protein levels of IkappaBalpha  and  p105 in the cytoplasm.	transcription
54793	5	335278	5	NULL	NULL	0	NULL	mitomycin C			does not affect					p105		protein levels of			NULL	cytoplasm	0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31244_s_7	8537390	In concomitance with NF-kappaB activation,  mitomycin C induced the processing of p105 to p50 in the nucleus, while  it did not affect the steady-state protein levels of IkappaBalpha  and  p105 in the cytoplasm.	transcription
55892	1	335278	7	NULL	NULL	0	NULL	p105			processed to					p50					NULL	nucleus	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31244_s_7	8537390	In concomitance with NF-kappaB activation,  mitomycin C induced the processing of p105 to p50 in the nucleus, while  it did not affect the steady-state protein levels of IkappaBalpha  and  p105 in the cytoplasm.	transcription
55893	2	335278	7	NULL	NULL	0	NULL	 mitomycin C			induce					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31244_s_7	8537390	In concomitance with NF-kappaB activation,  mitomycin C induced the processing of p105 to p50 in the nucleus, while  it did not affect the steady-state protein levels of IkappaBalpha  and  p105 in the cytoplasm.	transcription
55894	3	335278	7	NULL	NULL	0	NULL	statement 2			occurs upon					NF-kappaB		activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31244_s_7	8537390	In concomitance with NF-kappaB activation,  mitomycin C induced the processing of p105 to p50 in the nucleus, while  it did not affect the steady-state protein levels of IkappaBalpha  and  p105 in the cytoplasm.	transcription
55895	4	335278	7	NULL	NULL	0	NULL	mitomycin C			does not affect					IkappaBalpha		steady-state protein levels of 			NULL	cytoplasm	0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31244_s_7	8537390	In concomitance with NF-kappaB activation,  mitomycin C induced the processing of p105 to p50 in the nucleus, while  it did not affect the steady-state protein levels of IkappaBalpha  and  p105 in the cytoplasm.	transcription
55896	5	335278	7	NULL	NULL	0	NULL	mitomycin C			does not affect					p105		steady-state protein levels of			NULL	cytoplasm	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_52_31244_s_7	8537390	In concomitance with NF-kappaB activation,  mitomycin C induced the processing of p105 to p50 in the nucleus, while  it did not affect the steady-state protein levels of IkappaBalpha  and  p105 in the cytoplasm.	transcription
54794	1	335280	5	NULL	NULL	0	NULL	transactivation			is dependent on					NF-kappaB					NULL		0	NULL	NULL	NULL	gw70_jclininvest_114_10_1504_s_48	15546001	To investigate a potential role of p50 and Bcl-3 in this NF-kappaB - dependent transactivation during disuse atrophy, we studied mice with a knockout of  Nfkb1 (which encodes the p105 and p50 protein) or  Bcl3.	transcription
54795	2	335280	5	NULL	NULL	0	NULL	statement 1			occurs during					disuse atrophy					NULL		0	NULL	NULL	NULL	gw70_jclininvest_114_10_1504_s_48	15546001	To investigate a potential role of p50 and Bcl-3 in this NF-kappaB - dependent transactivation during disuse atrophy, we studied mice with a knockout of  Nfkb1 (which encodes the p105 and p50 protein) or  Bcl3.	transcription
54796	3	335280	5	NULL	NULL	0	NULL	p50			plays a role in		potentially			statement 1					NULL		0	NULL	NULL	NULL	gw70_jclininvest_114_10_1504_s_48	15546001	To investigate a potential role of p50 and Bcl-3 in this NF-kappaB - dependent transactivation during disuse atrophy, we studied mice with a knockout of  Nfkb1 (which encodes the p105 and p50 protein) or  Bcl3.	transcription
54797	4	335280	5	NULL	NULL	0	NULL	Bcl-3			plays a role in		potentially			statement 1					NULL		0	NULL	NULL	NULL	gw70_jclininvest_114_10_1504_s_48	15546001	To investigate a potential role of p50 and Bcl-3 in this NF-kappaB - dependent transactivation during disuse atrophy, we studied mice with a knockout of  Nfkb1 (which encodes the p105 and p50 protein) or  Bcl3.	transcription
54798	5	335280	5	NULL	NULL	0	NULL	Nfkb1			encodes					p105 protein					NULL		0	NULL	NULL	NULL	gw70_jclininvest_114_10_1504_s_48	15546001	To investigate a potential role of p50 and Bcl-3 in this NF-kappaB - dependent transactivation during disuse atrophy, we studied mice with a knockout of  Nfkb1 (which encodes the p105 and p50 protein) or  Bcl3.	transcription
54799	6	335280	5	NULL	NULL	0	NULL	Nfkb1			encodes					p50 protein					NULL		0	NULL	NULL	NULL	gw70_jclininvest_114_10_1504_s_48	15546001	To investigate a potential role of p50 and Bcl-3 in this NF-kappaB - dependent transactivation during disuse atrophy, we studied mice with a knockout of  Nfkb1 (which encodes the p105 and p50 protein) or  Bcl3.	transcription
56147	1	335280	7	NULL	NULL	0	NULL	Nfkb1			encode					p105					NULL		0	NULL	NULL	NULL	gw70_jclininvest_114_10_1504_s_48	15546001	To investigate a potential role of p50 and Bcl-3 in this NF-kappaB - dependent transactivation during disuse atrophy, we studied mice with a knockout of  Nfkb1 (which encodes the p105 and p50 protein) or  Bcl3.	transcription
56148	2	335280	7	NULL	NULL	0	NULL	Nfkb1			encode					p50 protein					NULL		0	NULL	NULL	NULL	gw70_jclininvest_114_10_1504_s_48	15546001	To investigate a potential role of p50 and Bcl-3 in this NF-kappaB - dependent transactivation during disuse atrophy, we studied mice with a knockout of  Nfkb1 (which encodes the p105 and p50 protein) or  Bcl3.	transcription
54800	1	335281	5	NULL	NULL	0	NULL	p50		newly synthesized	is encoded by					p50 expression vector					NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_165	9529257	However, newly synthesized p50 encoded by a p50  expression vector was effectively coimmunoprecipitated by the E446-1 antibody (lane 12), suggesting that  the interaction of p105 fragments with the proteasome may occur during translation.	transcription
54801	2	335281	5	NULL	NULL	0	NULL	E446-1 antibody			coimmunoprecipitates with		effectively			statement 1					NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_165	9529257	However, newly synthesized p50 encoded by a p50  expression vector was effectively coimmunoprecipitated by the E446-1 antibody (lane 12), suggesting that  the interaction of p105 fragments with the proteasome may occur during translation.	transcription
54802	3	335281	5	NULL	NULL	0	NULL	p105 fragments 			interacts with					proteasome					NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_165	9529257	However, newly synthesized p50 encoded by a p50  expression vector was effectively coimmunoprecipitated by the E446-1 antibody (lane 12), suggesting that  the interaction of p105 fragments with the proteasome may occur during translation.	transcription
54803	4	335281	5	NULL	NULL	0	NULL	statement 3			occurs during		may			translation					NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_165	9529257	However, newly synthesized p50 encoded by a p50  expression vector was effectively coimmunoprecipitated by the E446-1 antibody (lane 12), suggesting that  the interaction of p105 fragments with the proteasome may occur during translation.	transcription
55897	1	335281	7	NULL	NULL	0	NULL	p50		newly synthesized	bind					E446-1 antibody					NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_165	9529257	However, newly synthesized p50 encoded by a p50  expression vector was effectively coimmunoprecipitated by the E446-1 antibody (lane 12), suggesting that  the interaction of p105 fragments with the proteasome may occur during translation.	transcription
55898	2	335281	7	NULL	NULL	0	NULL	p105 fragments 			interacts with					proteasome					NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_165	9529257	However, newly synthesized p50 encoded by a p50  expression vector was effectively coimmunoprecipitated by the E446-1 antibody (lane 12), suggesting that  the interaction of p105 fragments with the proteasome may occur during translation.	transcription
55899	3	335281	7	NULL	NULL	0	NULL	statement 2			occur during		may			translation					NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_165	9529257	However, newly synthesized p50 encoded by a p50  expression vector was effectively coimmunoprecipitated by the E446-1 antibody (lane 12), suggesting that  the interaction of p105 fragments with the proteasome may occur during translation.	transcription
54804	1	335282	5	NULL	NULL	0	NULL	p105		proteolytic processing of	leads to					p50		nuclear translocation of			NULL	transfected 3T3cells	0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_65	9950430	To determine whether TPL-2 must induce proteolytic processing of p105 to promote nuclear translocation of p50, we transfected 3T3cells with a vector encoding Myc - p105deltaGRR 18, together with haemagglutinin (HA) - p50 on a separate plasmid.	transcription
54805	2	335282	5	NULL	NULL	0	NULL	TPL-2			induce		might			statement 1					NULL	transfected 3T3cells	NULL	NULL	NULL	NULL	gw60_nature_397_6717_363_s_65	9950430	To determine whether TPL-2 must induce proteolytic processing of p105 to promote nuclear translocation of p50, we transfected 3T3cells with a vector encoding Myc - p105deltaGRR 18, together with haemagglutinin (HA) - p50 on a separate plasmid.	transcription
56174	1	335282	7	NULL	NULL	0	NULL	p105		proteolytic processing of	promote					p50		nuclear translocation of 			NULL	transfected 3T3cells	0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_65	9950430	To determine whether TPL-2 must induce proteolytic processing of p105 to promote nuclear translocation of p50, we transfected 3T3cells with a vector encoding Myc - p105deltaGRR 18, together with haemagglutinin (HA) - p50 on a separate plasmid.	transcription
56175	2	335282	7	NULL	NULL	0	NULL	TPL-2			induce		might			statement 1					NULL	transfected 3T3cells	0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_65	9950430	To determine whether TPL-2 must induce proteolytic processing of p105 to promote nuclear translocation of p50, we transfected 3T3cells with a vector encoding Myc - p105deltaGRR 18, together with haemagglutinin (HA) - p50 on a separate plasmid.	transcription
54806	1	335284	5	NULL	NULL	0	NULL	NF-kappaB-1 p105			resides in			PEST sequence		NF-kappaB-1 p105			C-terminus		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_52_35201_s_220	9857058	Moreover, the C-terminal PEST sequence of NF-kappaB-1 p105 also plays an important role in its processing; it was shown by MacKichan  et al. ( 46) that phosphorylation of the PEST sequences of p105 up-regulates the proteolytic processing of p105 into the active p50.	transcription
54807	2	335284	5	NULL	NULL	0	NULL	statement 1			plays a role in					NF-kappaB-1 p105		processing of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_52_35201_s_220	9857058	Moreover, the C-terminal PEST sequence of NF-kappaB-1 p105 also plays an important role in its processing; it was shown by MacKichan  et al. ( 46) that phosphorylation of the PEST sequences of p105 up-regulates the proteolytic processing of p105 into the active p50.	transcription
54808	4	335284	5	NULL	NULL	0	NULL	NF-kappaB-1 p105		phosphorylation of	upregulates			PEST sequence		statement 3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_52_35201_s_220	9857058	Moreover, the C-terminal PEST sequence of NF-kappaB-1 p105 also plays an important role in its processing; it was shown by MacKichan  et al. ( 46) that phosphorylation of the PEST sequences of p105 up-regulates the proteolytic processing of p105 into the active p50.	transcription
54809	3	335284	5	NULL	NULL	0	NULL	p105		proteolytic processing of	forms					p50		active			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_52_35201_s_220	9857058	Moreover, the C-terminal PEST sequence of NF-kappaB-1 p105 also plays an important role in its processing; it was shown by MacKichan  et al. ( 46) that phosphorylation of the PEST sequences of p105 up-regulates the proteolytic processing of p105 into the active p50.	transcription
55900	1	335284	7	NULL	NULL	0	NULL	NF-kappaB-1 p105 			plays an important role in			C-terminal PEST sequence		NF-kappaB-1 p105 		processing of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_52_35201_s_220	9857058	Moreover, the C-terminal PEST sequence of NF-kappaB-1 p105 also plays an important role in its processing; it was shown by MacKichan  et al. ( 46) that phosphorylation of the PEST sequences of p105 up-regulates the proteolytic processing of p105 into the active p50.	transcription
55901	2	335284	7	NULL	NULL	0	NULL	p105 			processed to		proteolytically			p50		active			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_52_35201_s_220	9857058	Moreover, the C-terminal PEST sequence of NF-kappaB-1 p105 also plays an important role in its processing; it was shown by MacKichan  et al. ( 46) that phosphorylation of the PEST sequences of p105 up-regulates the proteolytic processing of p105 into the active p50.	transcription
55902	3	335284	7	NULL	NULL	0	NULL	p105		phosphorylation of 	upregulates			PEST sequences		statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_52_35201_s_220	9857058	Moreover, the C-terminal PEST sequence of NF-kappaB-1 p105 also plays an important role in its processing; it was shown by MacKichan  et al. ( 46) that phosphorylation of the PEST sequences of p105 up-regulates the proteolytic processing of p105 into the active p50.	transcription
54810	1	335285	5	NULL	NULL	0	NULL	BCL-3			is a type of					oncoprotein					NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_218	9529257	While the biological function of these  Rel-p105 complexes remains to be elucidated, the candidate oncoprotein BCL-3 may mobilize p50  molecules bound to p105 without enhancing p105 processing (Watanabe et al., 1997   ), suggesting that p105/p50 complexes could function as a source of p50 homodimers.	transcription
54811	2	335285	5	NULL	NULL	0	NULL	p50			bind					p105					NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_218	9529257	While the biological function of these  Rel-p105 complexes remains to be elucidated, the candidate oncoprotein BCL-3 may mobilize p50  molecules bound to p105 without enhancing p105 processing (Watanabe et al., 1997   ), suggesting that p105/p50 complexes could function as a source of p50 homodimers.	transcription
54812	3	335285	5	NULL	NULL	0	NULL	BCL-3			mobilize		may			statement 2					NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_218	9529257	While the biological function of these  Rel-p105 complexes remains to be elucidated, the candidate oncoprotein BCL-3 may mobilize p50  molecules bound to p105 without enhancing p105 processing (Watanabe et al., 1997   ), suggesting that p105/p50 complexes could function as a source of p50 homodimers.	transcription
54813	4	335285	5	NULL	NULL	0	NULL	statement 3			does not enhance					p105		processing of			NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_218	9529257	While the biological function of these  Rel-p105 complexes remains to be elucidated, the candidate oncoprotein BCL-3 may mobilize p50  molecules bound to p105 without enhancing p105 processing (Watanabe et al., 1997   ), suggesting that p105/p50 complexes could function as a source of p50 homodimers.	transcription
54814	5	335285	5	NULL	NULL	0	NULL	p105/p50 complexes			function as		may			p50 homodimers		source of			NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_218	9529257	While the biological function of these  Rel-p105 complexes remains to be elucidated, the candidate oncoprotein BCL-3 may mobilize p50  molecules bound to p105 without enhancing p105 processing (Watanabe et al., 1997   ), suggesting that p105/p50 complexes could function as a source of p50 homodimers.	transcription
55903	1	335285	7	NULL	NULL	0	NULL	p50 molecules			bind					p105					NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_218	9529257	While the biological function of these  Rel-p105 complexes remains to be elucidated, the candidate oncoprotein BCL-3 may mobilize p50  molecules bound to p105 without enhancing p105 processing (Watanabe et al., 1997   ), suggesting that p105/p50 complexes could function as a source of p50 homodimers.	transcription
55904	2	335285	7	NULL	NULL	0	NULL	BCL-3 			mobilize		may			statement 1					NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_218	9529257	While the biological function of these  Rel-p105 complexes remains to be elucidated, the candidate oncoprotein BCL-3 may mobilize p50  molecules bound to p105 without enhancing p105 processing (Watanabe et al., 1997   ), suggesting that p105/p50 complexes could function as a source of p50 homodimers.	transcription
55905	3	335285	7	NULL	NULL	0	NULL	statement 2			occurs without					p105		enhancing;;processing of			NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_218	9529257	While the biological function of these  Rel-p105 complexes remains to be elucidated, the candidate oncoprotein BCL-3 may mobilize p50  molecules bound to p105 without enhancing p105 processing (Watanabe et al., 1997   ), suggesting that p105/p50 complexes could function as a source of p50 homodimers.	transcription
55906	4	335285	7	NULL	NULL	0	NULL	p105/p50 complexes			function as					p50 homodimers		source of			NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_218	9529257	While the biological function of these  Rel-p105 complexes remains to be elucidated, the candidate oncoprotein BCL-3 may mobilize p50  molecules bound to p105 without enhancing p105 processing (Watanabe et al., 1997   ), suggesting that p105/p50 complexes could function as a source of p50 homodimers.	transcription
55907	5	335285	7	NULL	NULL	0	NULL	statement 3			suggest					statement 4					NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_218	9529257	While the biological function of these  Rel-p105 complexes remains to be elucidated, the candidate oncoprotein BCL-3 may mobilize p50  molecules bound to p105 without enhancing p105 processing (Watanabe et al., 1997   ), suggesting that p105/p50 complexes could function as a source of p50 homodimers.	transcription
55908	6	335285	7	NULL	NULL	0	NULL	BCL-3			is a type of					oncoprotein					NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_218	9529257	While the biological function of these  Rel-p105 complexes remains to be elucidated, the candidate oncoprotein BCL-3 may mobilize p50  molecules bound to p105 without enhancing p105 processing (Watanabe et al., 1997   ), suggesting that p105/p50 complexes could function as a source of p50 homodimers.	transcription
54815	1	335286	5	NULL	NULL	0	NULL	IKKbeta		expression of;;wild-type	increases					p50					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_226	11158290	While expression of wild-type IKKbeta led to increased p50, presumably by increasing p105 expression and concomitant p105 degradation, inactive IKKbeta reduced the amounts of p50 (Fig.  6B, left panel, compare lane 1 with 2 and 3).	transcription
54816	2	335286	5	NULL	NULL	0	NULL	IKKbeta		expression of;;wild-type	increases					p105		expression of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_226	11158290	While expression of wild-type IKKbeta led to increased p50, presumably by increasing p105 expression and concomitant p105 degradation, inactive IKKbeta reduced the amounts of p50 (Fig.  6B, left panel, compare lane 1 with 2 and 3).	transcription
54817	3	335286	5	NULL	NULL	0	NULL	statement 2			is concomitant to					p105		degradation of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_226	11158290	While expression of wild-type IKKbeta led to increased p50, presumably by increasing p105 expression and concomitant p105 degradation, inactive IKKbeta reduced the amounts of p50 (Fig.  6B, left panel, compare lane 1 with 2 and 3).	transcription
54826	4	335286	5	NULL	NULL	0	NULL	statement 2			leads to					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_226	11158290	While expression of wild-type IKKbeta led to increased p50, presumably by increasing p105 expression and concomitant p105 degradation, inactive IKKbeta reduced the amounts of p50 (Fig.  6B, left panel, compare lane 1 with 2 and 3).	transcription
54827	5	335286	5	NULL	NULL	0	NULL	statement 3			leads to					statement 1					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_226	11158290	While expression of wild-type IKKbeta led to increased p50, presumably by increasing p105 expression and concomitant p105 degradation, inactive IKKbeta reduced the amounts of p50 (Fig.  6B, left panel, compare lane 1 with 2 and 3).	transcription
54828	6	335286	5	NULL	NULL	0	NULL	IKKbeta		inactive	reduces					p50		amounts of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_226	11158290	While expression of wild-type IKKbeta led to increased p50, presumably by increasing p105 expression and concomitant p105 degradation, inactive IKKbeta reduced the amounts of p50 (Fig.  6B, left panel, compare lane 1 with 2 and 3).	transcription
55909	1	335286	7	NULL	NULL	0	NULL	IKKbeta		 expression of wild-type	increased					p50					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_226	11158290	While expression of wild-type IKKbeta led to increased p50, presumably by increasing p105 expression and concomitant p105 degradation, inactive IKKbeta reduced the amounts of p50 (Fig.  6B, left panel, compare lane 1 with 2 and 3).	transcription
55910	2	335286	7	NULL	NULL	0	NULL	statement 1			occur by increasing		presumably			p105		expression of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_226	11158290	While expression of wild-type IKKbeta led to increased p50, presumably by increasing p105 expression and concomitant p105 degradation, inactive IKKbeta reduced the amounts of p50 (Fig.  6B, left panel, compare lane 1 with 2 and 3).	transcription
55911	3	335286	7	NULL	NULL	0	NULL	statement 1			occur by increasing					p105		degradation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_226	11158290	While expression of wild-type IKKbeta led to increased p50, presumably by increasing p105 expression and concomitant p105 degradation, inactive IKKbeta reduced the amounts of p50 (Fig.  6B, left panel, compare lane 1 with 2 and 3).	transcription
55912	4	335286	7	NULL	NULL	0	NULL	IKKbeta		inactive	reduce					p50		amount of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_226	11158290	While expression of wild-type IKKbeta led to increased p50, presumably by increasing p105 expression and concomitant p105 degradation, inactive IKKbeta reduced the amounts of p50 (Fig.  6B, left panel, compare lane 1 with 2 and 3).	transcription
54829	1	335287	5	NULL	NULL	0	NULL	p105 precursor protein		phosphorylation of	is dependent on					IKK					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_13_11116_s_197	11799112	Because p50 activity is regulated predominantly through IKK-dependent phosphorylation and proteolysis of the p105 precursor protein ( 49-51), we analyzed whether PTEN blocked p50 activity by inhibiting p105 processing in LNCaP cells following TNF stimulation.	transcription
54830	2	335287	5	NULL	NULL	0	NULL	p105 precursor protein		proteolysis of	is dependent on					IKK					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_13_11116_s_197	11799112	Because p50 activity is regulated predominantly through IKK-dependent phosphorylation and proteolysis of the p105 precursor protein ( 49-51), we analyzed whether PTEN blocked p50 activity by inhibiting p105 processing in LNCaP cells following TNF stimulation.	transcription
54831	3	335287	5	NULL	NULL	0	NULL	p50		activity of	is regulated through		predominantly			statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_13_11116_s_197	11799112	Because p50 activity is regulated predominantly through IKK-dependent phosphorylation and proteolysis of the p105 precursor protein ( 49-51), we analyzed whether PTEN blocked p50 activity by inhibiting p105 processing in LNCaP cells following TNF stimulation.	transcription
54832	4	335287	5	NULL	NULL	0	NULL	p50		activity of	is regulated through		predominantly			statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_13_11116_s_197	11799112	Because p50 activity is regulated predominantly through IKK-dependent phosphorylation and proteolysis of the p105 precursor protein ( 49-51), we analyzed whether PTEN blocked p50 activity by inhibiting p105 processing in LNCaP cells following TNF stimulation.	transcription
54833	5	335287	5	NULL	NULL	0	NULL	PTEN			block		potentially			p50		activity of			NULL	LNCaP cells	0	NULL	NULL	NULL	gw60_jbiolchem_277_13_11116_s_197	11799112	Because p50 activity is regulated predominantly through IKK-dependent phosphorylation and proteolysis of the p105 precursor protein ( 49-51), we analyzed whether PTEN blocked p50 activity by inhibiting p105 processing in LNCaP cells following TNF stimulation.	transcription
54834	6	335287	5	NULL	NULL	0	NULL	PTEN			inhibits		potentially			p105		degradation of			NULL	LNCaP cells	0	NULL	NULL	NULL	gw60_jbiolchem_277_13_11116_s_197	11799112	Because p50 activity is regulated predominantly through IKK-dependent phosphorylation and proteolysis of the p105 precursor protein ( 49-51), we analyzed whether PTEN blocked p50 activity by inhibiting p105 processing in LNCaP cells following TNF stimulation.	transcription
54835	7	335287	5	NULL	NULL	0	NULL	statement 5			leads to		potentially			statement 6					NULL	LNCaP cells	0	NULL	NULL	NULL	gw60_jbiolchem_277_13_11116_s_197	11799112	Because p50 activity is regulated predominantly through IKK-dependent phosphorylation and proteolysis of the p105 precursor protein ( 49-51), we analyzed whether PTEN blocked p50 activity by inhibiting p105 processing in LNCaP cells following TNF stimulation.	transcription
54836	8	335287	5	NULL	NULL	0	NULL	TNF		stimulation	leads to		potentially			statement 7					NULL	LNCaP cells	0	NULL	NULL	NULL	gw60_jbiolchem_277_13_11116_s_197	11799112	Because p50 activity is regulated predominantly through IKK-dependent phosphorylation and proteolysis of the p105 precursor protein ( 49-51), we analyzed whether PTEN blocked p50 activity by inhibiting p105 processing in LNCaP cells following TNF stimulation.	transcription
55913	1	335287	7	NULL	NULL	0	NULL	p50		activity of	regulated through		predominantly			IKK-dependent phosphorylation 					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_13_11116_s_197	11799112	Because p50 activity is regulated predominantly through IKK-dependent phosphorylation and proteolysis of the p105 precursor protein ( 49-51), we analyzed whether PTEN blocked p50 activity by inhibiting p105 processing in LNCaP cells following TNF stimulation.	transcription
55914	2	335287	7	NULL	NULL	0	NULL	p50		activity of	regulated through		predominantly			p105 precursor protein 		proteolysis of	49-51		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_13_11116_s_197	11799112	Because p50 activity is regulated predominantly through IKK-dependent phosphorylation and proteolysis of the p105 precursor protein ( 49-51), we analyzed whether PTEN blocked p50 activity by inhibiting p105 processing in LNCaP cells following TNF stimulation.	transcription
55926	3	335287	7	NULL	NULL	0	NULL	statement 1			occur along with					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_13_11116_s_197	11799112	Because p50 activity is regulated predominantly through IKK-dependent phosphorylation and proteolysis of the p105 precursor protein ( 49-51), we analyzed whether PTEN blocked p50 activity by inhibiting p105 processing in LNCaP cells following TNF stimulation.	transcription
56781	1	335288	5	NULL	NULL	0	NULL	SCFbeta-TrCP ubiquitin ligase		stimulated	is recruited to								IKK-mediated phosphorylation motif at the C-terminal domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23253_s_241	11953428	Following stimulation, the SCFbeta-TrCP ubiquitin ligase is recruited to the IKK-mediated phosphorylation motif at the C-terminal domain, leading to rapid polyubiquitination and subsequent processing/degradation of p105 with release of the docked p50 molecules and an additional p50 subunit released from processed p105 ( 11,  12,  22).	transcription
56782	2	335288	5	NULL	NULL	0	NULL	statement 1			leads to					p105		rapid polyubiquitination of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23253_s_241	11953428	Following stimulation, the SCFbeta-TrCP ubiquitin ligase is recruited to the IKK-mediated phosphorylation motif at the C-terminal domain, leading to rapid polyubiquitination and subsequent processing/degradation of p105 with release of the docked p50 molecules and an additional p50 subunit released from processed p105 ( 11,  12,  22).	transcription
56783	3	335288	5	NULL	NULL	0	NULL	statement 2			leads to		subsequently			p105		processing/degradation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23253_s_241	11953428	Following stimulation, the SCFbeta-TrCP ubiquitin ligase is recruited to the IKK-mediated phosphorylation motif at the C-terminal domain, leading to rapid polyubiquitination and subsequent processing/degradation of p105 with release of the docked p50 molecules and an additional p50 subunit released from processed p105 ( 11,  12,  22).	transcription
56784	4	335288	5	NULL	NULL	0	NULL	statement 3			release					p50 molecules		docked			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_26_23253_s_241	11953428	Following stimulation, the SCFbeta-TrCP ubiquitin ligase is recruited to the IKK-mediated phosphorylation motif at the C-terminal domain, leading to rapid polyubiquitination and subsequent processing/degradation of p105 with release of the docked p50 molecules and an additional p50 subunit released from processed p105 ( 11,  12,  22).	transcription
56785	5	335288	5	NULL	NULL	0	NULL	p50 subunit			is relased from					p105		processed			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23253_s_241	11953428	Following stimulation, the SCFbeta-TrCP ubiquitin ligase is recruited to the IKK-mediated phosphorylation motif at the C-terminal domain, leading to rapid polyubiquitination and subsequent processing/degradation of p105 with release of the docked p50 molecules and an additional p50 subunit released from processed p105 ( 11,  12,  22).	transcription
56786	6	335288	5	NULL	NULL	0	NULL	statement 3			leads to					statement 5					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23253_s_241	11953428	Following stimulation, the SCFbeta-TrCP ubiquitin ligase is recruited to the IKK-mediated phosphorylation motif at the C-terminal domain, leading to rapid polyubiquitination and subsequent processing/degradation of p105 with release of the docked p50 molecules and an additional p50 subunit released from processed p105 ( 11,  12,  22).	transcription
55915	1	335288	7	NULL	NULL	0	NULL	SCFbeta-TrCP ubiquitin ligase 			recruited to								IKK-mediated phosphorylation motif at the C-terminal domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23253_s_241	11953428	Following stimulation, the SCFbeta-TrCP ubiquitin ligase is recruited to the IKK-mediated phosphorylation motif at the C-terminal domain, leading to rapid polyubiquitination and subsequent processing/degradation of p105 with release of the docked p50 molecules and an additional p50 subunit released from processed p105 ( 11,  12,  22).	transcription
55916	2	335288	7	NULL	NULL	0	NULL	statement 1			leads to		rapidly			polyubiquitination					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23253_s_241	11953428	Following stimulation, the SCFbeta-TrCP ubiquitin ligase is recruited to the IKK-mediated phosphorylation motif at the C-terminal domain, leading to rapid polyubiquitination and subsequent processing/degradation of p105 with release of the docked p50 molecules and an additional p50 subunit released from processed p105 ( 11,  12,  22).	transcription
55917	3	335288	7	NULL	NULL	0	NULL	statement 1			leads to		rapidly			p105		processing/degradation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23253_s_241	11953428	Following stimulation, the SCFbeta-TrCP ubiquitin ligase is recruited to the IKK-mediated phosphorylation motif at the C-terminal domain, leading to rapid polyubiquitination and subsequent processing/degradation of p105 with release of the docked p50 molecules and an additional p50 subunit released from processed p105 ( 11,  12,  22).	transcription
55918	4	335288	7	NULL	NULL	0	NULL	statement 3			release					p50 molecules 		docked			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23253_s_241	11953428	Following stimulation, the SCFbeta-TrCP ubiquitin ligase is recruited to the IKK-mediated phosphorylation motif at the C-terminal domain, leading to rapid polyubiquitination and subsequent processing/degradation of p105 with release of the docked p50 molecules and an additional p50 subunit released from processed p105 ( 11,  12,  22).	transcription
55919	5	335288	7	NULL	NULL	0	NULL	p50 subunit			released from					p105		processed			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23253_s_241	11953428	Following stimulation, the SCFbeta-TrCP ubiquitin ligase is recruited to the IKK-mediated phosphorylation motif at the C-terminal domain, leading to rapid polyubiquitination and subsequent processing/degradation of p105 with release of the docked p50 molecules and an additional p50 subunit released from processed p105 ( 11,  12,  22).	transcription
55920	6	335288	7	NULL	NULL	0	NULL	statement 3			leads to					statement 5					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23253_s_241	11953428	Following stimulation, the SCFbeta-TrCP ubiquitin ligase is recruited to the IKK-mediated phosphorylation motif at the C-terminal domain, leading to rapid polyubiquitination and subsequent processing/degradation of p105 with release of the docked p50 molecules and an additional p50 subunit released from processed p105 ( 11,  12,  22).	transcription
55921	7	335288	7	NULL	NULL	0	NULL	statement 1			occur upon					stimulation					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23253_s_241	11953428	Following stimulation, the SCFbeta-TrCP ubiquitin ligase is recruited to the IKK-mediated phosphorylation motif at the C-terminal domain, leading to rapid polyubiquitination and subsequent processing/degradation of p105 with release of the docked p50 molecules and an additional p50 subunit released from processed p105 ( 11,  12,  22).	transcription
54845	1	335289	5	NULL	NULL	0	NULL	LTbetaR		signaling of	induces					p105 precursor		processingof;;degradation of 			NULL		0	NULL	NULL	NULL	gw70_embo_22_1_121_s_224	12505990	We observed that LTbetaR signaling also induces processing/degradation of the p105 precursor with similar  kinetics to p100, but without altering p50 levels.	transcription
54846	2	335289	5	NULL	NULL	0	NULL	statement 1			does not alter					p50		levels of			NULL		0	NULL	NULL	NULL	gw70_embo_22_1_121_s_224	12505990	We observed that LTbetaR signaling also induces processing/degradation of the p105 precursor with similar  kinetics to p100, but without altering p50 levels.	transcription
54847	3	335289	5	NULL	NULL	0	NULL	LTbetaR		signaling of	induces					p100		processingof;;degradation of			NULL		0	NULL	NULL	NULL	gw70_embo_22_1_121_s_224	12505990	We observed that LTbetaR signaling also induces processing/degradation of the p105 precursor with similar  kinetics to p100, but without altering p50 levels.	transcription
54848	4	335289	5	NULL	NULL	0	NULL	statement 1		kinetics of	similar to					statement 3		kinetics of			NULL		0	NULL	NULL	NULL	gw70_embo_22_1_121_s_224	12505990	We observed that LTbetaR signaling also induces processing/degradation of the p105 precursor with similar  kinetics to p100, but without altering p50 levels.	transcription
55922	1	335289	7	NULL	NULL	0	NULL	 LTbetaR 		signaling of	induce					p105 precursor		processing/degradation of			NULL		NULL	NULL	NULL	NULL	gw70_embo_22_1_121_s_224	12505990	We observed that LTbetaR signaling also induces processing/degradation of the p105 precursor with similar  kinetics to p100, but without altering p50 levels.	transcription
55923	2	335289	7	NULL	NULL	0	NULL	LTbetaR		signaling of	induce					p100		processing/degradation of			NULL		0	NULL	NULL	NULL	gw70_embo_22_1_121_s_224	12505990	We observed that LTbetaR signaling also induces processing/degradation of the p105 precursor with similar  kinetics to p100, but without altering p50 levels.	transcription
55924	3	335289	7	NULL	NULL	0	NULL	statement 1			does not alter					p50		levels of			NULL		0	NULL	NULL	NULL	gw70_embo_22_1_121_s_224	12505990	We observed that LTbetaR signaling also induces processing/degradation of the p105 precursor with similar  kinetics to p100, but without altering p50 levels.	transcription
55925	4	335289	7	NULL	NULL	0	NULL	statement 2			does not alter					p50		levels of			NULL		0	NULL	NULL	NULL	gw70_embo_22_1_121_s_224	12505990	We observed that LTbetaR signaling also induces processing/degradation of the p105 precursor with similar  kinetics to p100, but without altering p50 levels.	transcription
54849	1	335290	5	NULL	NULL	0	NULL	p105			is a precursor of					p50					NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_27_9_1883_s_257	16624828	1,25-VD has been shown to reduce levels of p50 and its precursor p105 and then decrease PMA-induced NF-kappaB binding to the IL-6promoter in human lymphocytes ( ).	transcription
54850	2	335290	5	NULL	NULL	0	NULL	1,25-VD			reduces					p50		levels of			NULL	human lymphocytes	NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_9_1883_s_257	16624828	1,25-VD has been shown to reduce levels of p50 and its precursor p105 and then decrease PMA-induced NF-kappaB binding to the IL-6promoter in human lymphocytes ( ).	transcription
54851	3	335290	5	NULL	NULL	0	NULL	1,25-VD			reduces					p105		levels of			NULL	human lymphocytes	NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_9_1883_s_257	16624828	1,25-VD has been shown to reduce levels of p50 and its precursor p105 and then decrease PMA-induced NF-kappaB binding to the IL-6promoter in human lymphocytes ( ).	transcription
54852	4	335290	5	NULL	NULL	0	NULL	NF-kappaB			bind					IL-6				promoter	NULL	human lymphocytes	0	NULL	NULL	NULL	gw70_carcinogenesis_27_9_1883_s_257	16624828	1,25-VD has been shown to reduce levels of p50 and its precursor p105 and then decrease PMA-induced NF-kappaB binding to the IL-6promoter in human lymphocytes ( ).	transcription
54853	5	335290	5	NULL	NULL	0	NULL	PMA			induces					statement 4					NULL	human lymphocytes	0	NULL	NULL	NULL	gw70_carcinogenesis_27_9_1883_s_257	16624828	1,25-VD has been shown to reduce levels of p50 and its precursor p105 and then decrease PMA-induced NF-kappaB binding to the IL-6promoter in human lymphocytes ( ).	transcription
54854	6	335290	5	NULL	NULL	0	NULL	1,25-VD			decreases					statement 5					NULL	human lymphocytes	0	NULL	NULL	NULL	gw70_carcinogenesis_27_9_1883_s_257	16624828	1,25-VD has been shown to reduce levels of p50 and its precursor p105 and then decrease PMA-induced NF-kappaB binding to the IL-6promoter in human lymphocytes ( ).	transcription
54855	7	335290	5	NULL	NULL	0	NULL	statement 2			leads to					statement 6					NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_27_9_1883_s_257	16624828	1,25-VD has been shown to reduce levels of p50 and its precursor p105 and then decrease PMA-induced NF-kappaB binding to the IL-6promoter in human lymphocytes ( ).	transcription
54856	8	335290	5	NULL	NULL	0	NULL	statement 3			leads to					statement 6					NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_27_9_1883_s_257	16624828	1,25-VD has been shown to reduce levels of p50 and its precursor p105 and then decrease PMA-induced NF-kappaB binding to the IL-6promoter in human lymphocytes ( ).	transcription
55927	1	335290	7	NULL	NULL	0	NULL	1,25-VD 			reduce					p50		levels of			NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_27_9_1883_s_257	16624828	1,25-VD has been shown to reduce levels of p50 and its precursor p105 and then decrease PMA-induced NF-kappaB binding to the IL-6promoter in human lymphocytes ( ).	transcription
55928	2	335290	7	NULL	NULL	0	NULL	1,25-VD 			reduce					p105		levels of			NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_9_1883_s_257	16624828	1,25-VD has been shown to reduce levels of p50 and its precursor p105 and then decrease PMA-induced NF-kappaB binding to the IL-6promoter in human lymphocytes ( ).	transcription
55929	3	335290	7	NULL	NULL	0	NULL	NF-kappaB			bind					IL-6				promoter	NULL	human lymphocytes	0	NULL	NULL	NULL	gw70_carcinogenesis_27_9_1883_s_257	16624828	1,25-VD has been shown to reduce levels of p50 and its precursor p105 and then decrease PMA-induced NF-kappaB binding to the IL-6promoter in human lymphocytes ( ).	transcription
55930	4	335290	7	NULL	NULL	0	NULL	PMA			induce					statement 3					NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_27_9_1883_s_257	16624828	1,25-VD has been shown to reduce levels of p50 and its precursor p105 and then decrease PMA-induced NF-kappaB binding to the IL-6promoter in human lymphocytes ( ).	transcription
55931	5	335290	7	NULL	NULL	0	NULL	1,25-VD			decrease					statement 4					NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_27_9_1883_s_257	16624828	1,25-VD has been shown to reduce levels of p50 and its precursor p105 and then decrease PMA-induced NF-kappaB binding to the IL-6promoter in human lymphocytes ( ).	transcription
54857	1	335292	5	NULL	NULL	0	NULL	IKK			mediates					p105		phosphorylation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8460_s_282	14668329	Signal-induced degradation of p105 could result from IKK-mediated phosphorylation and targeting by the proteasome ( ,  ,  ); then released p50 might be sequestered and transported to the nucleus by Bcl-3.	transcription
54858	2	335292	5	NULL	NULL	0	NULL	p105			is targeted by					proteasome					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8460_s_282	14668329	Signal-induced degradation of p105 could result from IKK-mediated phosphorylation and targeting by the proteasome ( ,  ,  ); then released p50 might be sequestered and transported to the nucleus by Bcl-3.	transcription
54859	3	335292	5	NULL	NULL	0	NULL	statement 1			leads to					statement 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8460_s_282	14668329	Signal-induced degradation of p105 could result from IKK-mediated phosphorylation and targeting by the proteasome ( ,  ,  ); then released p50 might be sequestered and transported to the nucleus by Bcl-3.	transcription
54860	4	335292	5	NULL	NULL	0	NULL	statement 3			results in					p105		degradation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8460_s_282	14668329	Signal-induced degradation of p105 could result from IKK-mediated phosphorylation and targeting by the proteasome ( ,  ,  ); then released p50 might be sequestered and transported to the nucleus by Bcl-3.	transcription
54861	5	335292	5	NULL	NULL	0	NULL	statement 4			releases					p50					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8460_s_282	14668329	Signal-induced degradation of p105 could result from IKK-mediated phosphorylation and targeting by the proteasome ( ,  ,  ); then released p50 might be sequestered and transported to the nucleus by Bcl-3.	transcription
54862	6	335292	5	NULL	NULL	0	NULL	p50		released	undergoes					sequestration					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_8460_s_282	14668329	Signal-induced degradation of p105 could result from IKK-mediated phosphorylation and targeting by the proteasome ( ,  ,  ); then released p50 might be sequestered and transported to the nucleus by Bcl-3.	transcription
54863	7	335292	5	NULL	NULL	0	NULL	p50			is transported to					nucleus					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8460_s_282	14668329	Signal-induced degradation of p105 could result from IKK-mediated phosphorylation and targeting by the proteasome ( ,  ,  ); then released p50 might be sequestered and transported to the nucleus by Bcl-3.	transcription
54864	8	335292	5	NULL	NULL	0	NULL	Bcl-3			is required for					statement 7					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8460_s_282	14668329	Signal-induced degradation of p105 could result from IKK-mediated phosphorylation and targeting by the proteasome ( ,  ,  ); then released p50 might be sequestered and transported to the nucleus by Bcl-3.	transcription
55955	1	335292	7	NULL	NULL	0	NULL	Signal			induce					p105		degradation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8460_s_282	14668329	Signal-induced degradation of p105 could result from IKK-mediated phosphorylation and targeting by the proteasome ( ,  ,  ); then released p50 might be sequestered and transported to the nucleus by Bcl-3.	transcription
55956	2	335292	7	NULL	NULL	0	NULL	IKK			mediate					phosphorylation					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8460_s_282	14668329	Signal-induced degradation of p105 could result from IKK-mediated phosphorylation and targeting by the proteasome ( ,  ,  ); then released p50 might be sequestered and transported to the nucleus by Bcl-3.	transcription
55957	3	335292	7	NULL	NULL	0	NULL	statement 1			result from					statement 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8460_s_282	14668329	Signal-induced degradation of p105 could result from IKK-mediated phosphorylation and targeting by the proteasome ( ,  ,  ); then released p50 might be sequestered and transported to the nucleus by Bcl-3.	transcription
55958	4	335292	7	NULL	NULL	0	NULL	statement 1			result from					proteasome		targeting by			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8460_s_282	14668329	Signal-induced degradation of p105 could result from IKK-mediated phosphorylation and targeting by the proteasome ( ,  ,  ); then released p50 might be sequestered and transported to the nucleus by Bcl-3.	transcription
55959	5	335292	7	NULL	NULL	0	NULL	statement 3			occur along with					statement 4					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8460_s_282	14668329	Signal-induced degradation of p105 could result from IKK-mediated phosphorylation and targeting by the proteasome ( ,  ,  ); then released p50 might be sequestered and transported to the nucleus by Bcl-3.	transcription
55960	6	335292	7	NULL	NULL	0	NULL	Bcl-3			sequester		may			p50					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_8460_s_282	14668329	Signal-induced degradation of p105 could result from IKK-mediated phosphorylation and targeting by the proteasome ( ,  ,  ); then released p50 might be sequestered and transported to the nucleus by Bcl-3.	transcription
55961	7	335292	7	NULL	NULL	0	NULL	p50			be transpored to		may			nucleus					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_8460_s_282	14668329	Signal-induced degradation of p105 could result from IKK-mediated phosphorylation and targeting by the proteasome ( ,  ,  ); then released p50 might be sequestered and transported to the nucleus by Bcl-3.	transcription
55962	8	335292	7	NULL	NULL	0	NULL	Bcl-3			support					statement 7					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8460_s_282	14668329	Signal-induced degradation of p105 could result from IKK-mediated phosphorylation and targeting by the proteasome ( ,  ,  ); then released p50 might be sequestered and transported to the nucleus by Bcl-3.	transcription
54865	1	335293	5	NULL	NULL	0	NULL	NF-kappaB			is a family of					transcription factors					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_36_26041_s_30	16835236	NF-kappaB is a family of transcription factors that includes RelA (p65), NF-kappaB1 (p50 and p105), NF-kappaB2 (p52 and p100), c-Rel, and RelB.	transcription
54926	2	335293	5	NULL	NULL	0	NULL	statement 1			includes					RelA					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_36_26041_s_30	16835236	NF-kappaB is a family of transcription factors that includes RelA (p65), NF-kappaB1 (p50 and p105), NF-kappaB2 (p52 and p100), c-Rel, and RelB.	transcription
54927	3	335293	5	NULL	NULL	0	NULL	statement 1			includes					NF-kappaB1 p50					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_36_26041_s_30	16835236	NF-kappaB is a family of transcription factors that includes RelA (p65), NF-kappaB1 (p50 and p105), NF-kappaB2 (p52 and p100), c-Rel, and RelB.	transcription
54928	4	335293	5	NULL	NULL	0	NULL	statement 1			includes					NF-kappaB1 p105					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_36_26041_s_30	16835236	NF-kappaB is a family of transcription factors that includes RelA (p65), NF-kappaB1 (p50 and p105), NF-kappaB2 (p52 and p100), c-Rel, and RelB.	transcription
54929	5	335293	5	NULL	NULL	0	NULL	statement 1			includes					NF-kappaB2 p52					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_36_26041_s_30	16835236	NF-kappaB is a family of transcription factors that includes RelA (p65), NF-kappaB1 (p50 and p105), NF-kappaB2 (p52 and p100), c-Rel, and RelB.	transcription
54930	6	335293	5	NULL	NULL	0	NULL	statement 1			includes					NF-kappaB2 p100					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_36_26041_s_30	16835236	NF-kappaB is a family of transcription factors that includes RelA (p65), NF-kappaB1 (p50 and p105), NF-kappaB2 (p52 and p100), c-Rel, and RelB.	transcription
54931	7	335293	5	NULL	NULL	0	NULL	statement 1			includes					c-Rel					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_36_26041_s_30	16835236	NF-kappaB is a family of transcription factors that includes RelA (p65), NF-kappaB1 (p50 and p105), NF-kappaB2 (p52 and p100), c-Rel, and RelB.	transcription
54932	8	335293	5	NULL	NULL	0	NULL	statement 1			includes					RelB					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_36_26041_s_30	16835236	NF-kappaB is a family of transcription factors that includes RelA (p65), NF-kappaB1 (p50 and p105), NF-kappaB2 (p52 and p100), c-Rel, and RelB.	transcription
54933	9	335293	5	NULL	NULL	0	NULL	RelA			is a synonym of					p65					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_36_26041_s_30	16835236	NF-kappaB is a family of transcription factors that includes RelA (p65), NF-kappaB1 (p50 and p105), NF-kappaB2 (p52 and p100), c-Rel, and RelB.	transcription
55963	1	335293	7	NULL	NULL	0	NULL	NF-kappaB 			is a type of					transcription factors					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_36_26041_s_30	16835236	NF-kappaB is a family of transcription factors that includes RelA (p65), NF-kappaB1 (p50 and p105), NF-kappaB2 (p52 and p100), c-Rel, and RelB.	transcription
55964	2	335293	7	NULL	NULL	0	NULL	NF-kappaB family			include					RelA					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_36_26041_s_30	16835236	NF-kappaB is a family of transcription factors that includes RelA (p65), NF-kappaB1 (p50 and p105), NF-kappaB2 (p52 and p100), c-Rel, and RelB.	transcription
55965	3	335293	7	NULL	NULL	0	NULL	NF-kappaB family			include					NF-kappaB1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_36_26041_s_30	16835236	NF-kappaB is a family of transcription factors that includes RelA (p65), NF-kappaB1 (p50 and p105), NF-kappaB2 (p52 and p100), c-Rel, and RelB.	transcription
55966	4	335293	7	NULL	NULL	0	NULL	NF-kappaB family			include					NF-kappaB2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_36_26041_s_30	16835236	NF-kappaB is a family of transcription factors that includes RelA (p65), NF-kappaB1 (p50 and p105), NF-kappaB2 (p52 and p100), c-Rel, and RelB.	transcription
55967	5	335293	7	NULL	NULL	0	NULL	NF-kappaB family			include					c-Rel					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_36_26041_s_30	16835236	NF-kappaB is a family of transcription factors that includes RelA (p65), NF-kappaB1 (p50 and p105), NF-kappaB2 (p52 and p100), c-Rel, and RelB.	transcription
55968	6	335293	7	NULL	NULL	0	NULL	NF-kappaB family			include					RelB					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_36_26041_s_30	16835236	NF-kappaB is a family of transcription factors that includes RelA (p65), NF-kappaB1 (p50 and p105), NF-kappaB2 (p52 and p100), c-Rel, and RelB.	transcription
55969	7	335293	7	NULL	NULL	0	NULL	RelA 			is					p65					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_36_26041_s_30	16835236	NF-kappaB is a family of transcription factors that includes RelA (p65), NF-kappaB1 (p50 and p105), NF-kappaB2 (p52 and p100), c-Rel, and RelB.	transcription
55970	8	335293	7	NULL	NULL	0	NULL	NF-kappaB1			include					p50					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_36_26041_s_30	16835236	NF-kappaB is a family of transcription factors that includes RelA (p65), NF-kappaB1 (p50 and p105), NF-kappaB2 (p52 and p100), c-Rel, and RelB.	transcription
55971	9	335293	7	NULL	NULL	0	NULL	NF-kappaB1			include					p105					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_36_26041_s_30	16835236	NF-kappaB is a family of transcription factors that includes RelA (p65), NF-kappaB1 (p50 and p105), NF-kappaB2 (p52 and p100), c-Rel, and RelB.	transcription
55972	10	335293	7	NULL	NULL	0	NULL	NF-kappaB2 			include					p52					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_36_26041_s_30	16835236	NF-kappaB is a family of transcription factors that includes RelA (p65), NF-kappaB1 (p50 and p105), NF-kappaB2 (p52 and p100), c-Rel, and RelB.	transcription
55973	11	335293	7	NULL	NULL	0	NULL	NF-kappaB2 			include					p100					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_36_26041_s_30	16835236	NF-kappaB is a family of transcription factors that includes RelA (p65), NF-kappaB1 (p50 and p105), NF-kappaB2 (p52 and p100), c-Rel, and RelB.	transcription
54866	1	335294	5	NULL	NULL	0	NULL	gp 10		bacteriophage T7	is a type of					capsid protein					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_148	12807880	Replacement of a large  portion of p105 starting from the end of the GRR with either IkappaBalpha  or bacteriophage T7 capsid protein gp 10 does not affect p50  production ( ).	transcription
54867	2	335294	5	NULL	NULL	0	NULL	p105		large portion of	is replaced with					IkappaBalpha					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_148	12807880	Replacement of a large  portion of p105 starting from the end of the GRR with either IkappaBalpha  or bacteriophage T7 capsid protein gp 10 does not affect p50  production ( ).	transcription
54868	3	335294	5	NULL	NULL	0	NULL	p105		large portion of	is replaced with					gp 10		bacteriophage T7			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_148	12807880	Replacement of a large  portion of p105 starting from the end of the GRR with either IkappaBalpha  or bacteriophage T7 capsid protein gp 10 does not affect p50  production ( ).	transcription
54869	4	335294	5	NULL	NULL	0	NULL	statement 2			is an alternative to					statement 3					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_148	12807880	Replacement of a large  portion of p105 starting from the end of the GRR with either IkappaBalpha  or bacteriophage T7 capsid protein gp 10 does not affect p50  production ( ).	transcription
54870	5	335294	5	NULL	NULL	0	NULL	statement 2			does not affect					p50		production of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_148	12807880	Replacement of a large  portion of p105 starting from the end of the GRR with either IkappaBalpha  or bacteriophage T7 capsid protein gp 10 does not affect p50  production ( ).	transcription
54871	6	335294	5	NULL	NULL	0	NULL	statement 3			does not affect					p50		production of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_148	12807880	Replacement of a large  portion of p105 starting from the end of the GRR with either IkappaBalpha  or bacteriophage T7 capsid protein gp 10 does not affect p50  production ( ).	transcription
55974	1	335294	7	NULL	NULL	0	NULL	 IkappaBalpha			replace					p105 			 large portion from the end of GRR		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_148	12807880	Replacement of a large  portion of p105 starting from the end of the GRR with either IkappaBalpha  or bacteriophage T7 capsid protein gp 10 does not affect p50  production ( ).	transcription
55975	2	335294	7	NULL	NULL	0	NULL	gp 10			replace					p105 			large portion from the end of the GRR		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_148	12807880	Replacement of a large  portion of p105 starting from the end of the GRR with either IkappaBalpha  or bacteriophage T7 capsid protein gp 10 does not affect p50  production ( ).	transcription
55976	3	335294	7	NULL	NULL	0	NULL	gp 10			is a type of					 capsid protein		bacteriophage T7			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_148	12807880	Replacement of a large  portion of p105 starting from the end of the GRR with either IkappaBalpha  or bacteriophage T7 capsid protein gp 10 does not affect p50  production ( ).	transcription
55977	4	335294	7	NULL	NULL	0	NULL	statement 1			does not affect					p50		production of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_148	12807880	Replacement of a large  portion of p105 starting from the end of the GRR with either IkappaBalpha  or bacteriophage T7 capsid protein gp 10 does not affect p50  production ( ).	transcription
55978	5	335294	7	NULL	NULL	0	NULL	statement 2			does not affect					p50		production of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_148	12807880	Replacement of a large  portion of p105 starting from the end of the GRR with either IkappaBalpha  or bacteriophage T7 capsid protein gp 10 does not affect p50  production ( ).	transcription
54872	1	335295	5	NULL	NULL	0	NULL	p105 protein		proteolysis of	leads to					p50		production of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_196	12807880	Our work further confirmed that proteolysis leading to p50 production  initiates at an internal site, rather than at the C terminus of the p105  protein.	transcription
55979	1	335295	7	NULL	NULL	0	NULL	proteolysis			lead to					p50		production of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_196	12807880	Our work further confirmed that proteolysis leading to p50 production  initiates at an internal site, rather than at the C terminus of the p105  protein.	transcription
55980	2	335295	7	NULL	NULL	0	NULL	statement 1			initiates at an					internal site					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_196	12807880	Our work further confirmed that proteolysis leading to p50 production  initiates at an internal site, rather than at the C terminus of the p105  protein.	transcription
55981	3	335295	7	NULL	NULL	0	NULL	statement 1			does not initiate from					p105 			C terminus of		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_31479_s_196	12807880	Our work further confirmed that proteolysis leading to p50 production  initiates at an internal site, rather than at the C terminus of the p105  protein.	transcription
54873	1	335296	5	NULL	NULL	0	NULL	p105			is processed to					p50					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_41_39583_s_180	12871932	Indeed, some reports demonstrate that TNF-alpha induces p105 processing to p50 ( ,  ), others show that TNF-alpha induces complete degradation of the protein ( ,  ).	transcription
54874	2	335296	5	NULL	NULL	0	NULL	TNF-alpha			induces					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_41_39583_s_180	12871932	Indeed, some reports demonstrate that TNF-alpha induces p105 processing to p50 ( ,  ), others show that TNF-alpha induces complete degradation of the protein ( ,  ).	transcription
54875	3	335296	5	NULL	NULL	0	NULL	TNF-alpha			induces					p105		complete degradation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_41_39583_s_180	12871932	Indeed, some reports demonstrate that TNF-alpha induces p105 processing to p50 ( ,  ), others show that TNF-alpha induces complete degradation of the protein ( ,  ).	transcription
55982	1	335296	7	NULL	NULL	0	NULL	 p105			processed to					p50					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_41_39583_s_180	12871932	Indeed, some reports demonstrate that TNF-alpha induces p105 processing to p50 ( ,  ), others show that TNF-alpha induces complete degradation of the protein ( ,  ).	transcription
55983	2	335296	7	NULL	NULL	0	NULL	TNF-alpha			induce					statement 1					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_41_39583_s_180	12871932	Indeed, some reports demonstrate that TNF-alpha induces p105 processing to p50 ( ,  ), others show that TNF-alpha induces complete degradation of the protein ( ,  ).	transcription
55984	3	335296	7	NULL	NULL	0	NULL	 TNF-alpha			induce					p105		complete degradation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_41_39583_s_180	12871932	Indeed, some reports demonstrate that TNF-alpha induces p105 processing to p50 ( ,  ), others show that TNF-alpha induces complete degradation of the protein ( ,  ).	transcription
54876	1	335297	5	NULL	NULL	0	NULL	NFkappaB			is a precursor of			p105		NFkappaB			p50 subunit		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_48839_s_184	14514692	However, NFkappaB p105 is the precursor form of the NFkappaB p50 subunit that, in our study, did not appear to be the major subunit involved in the TNFalpha-dependent transcription of  MEFV.	transcription
54877	2	335297	5	NULL	NULL	0	NULL	MEFV		transcription of	is dependent on					TNFalpha					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_48839_s_184	14514692	However, NFkappaB p105 is the precursor form of the NFkappaB p50 subunit that, in our study, did not appear to be the major subunit involved in the TNFalpha-dependent transcription of  MEFV.	transcription
54878	3	335297	5	NULL	NULL	0	NULL	NFkappaB			not involved in		may	p105		statement 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_48839_s_184	14514692	However, NFkappaB p105 is the precursor form of the NFkappaB p50 subunit that, in our study, did not appear to be the major subunit involved in the TNFalpha-dependent transcription of  MEFV.	transcription
55985	1	335297	7	NULL	NULL	0	NULL	NFkappaB p105 			is precursor of					NFkappaB p50 subunit					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_48839_s_184	14514692	However, NFkappaB p105 is the precursor form of the NFkappaB p50 subunit that, in our study, did not appear to be the major subunit involved in the TNFalpha-dependent transcription of  MEFV.	transcription
55986	2	335297	7	NULL	NULL	0	NULL	MEFV		transcription of	depends on					 TNFalpha					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_48839_s_184	14514692	However, NFkappaB p105 is the precursor form of the NFkappaB p50 subunit that, in our study, did not appear to be the major subunit involved in the TNFalpha-dependent transcription of  MEFV.	transcription
55987	3	335297	7	NULL	NULL	0	NULL	 NFkappaB p50 subunit 			 not be involved in		may			statement 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_49_48839_s_184	14514692	However, NFkappaB p105 is the precursor form of the NFkappaB p50 subunit that, in our study, did not appear to be the major subunit involved in the TNFalpha-dependent transcription of  MEFV.	transcription
54879	1	335298	5	NULL	NULL	0	NULL	p105 inhibitor			gains					p50		early control of			NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_40	10970863	These results highlight a mechanism by which the p105 inhibitor gains very early control of the p50 transcription factor and provide a new perspective on Rel protein assembly.	transcription
54880	2	335298	5	NULL	NULL	0	NULL	p50			is a type of					transcription factor					NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_40	10970863	These results highlight a mechanism by which the p105 inhibitor gains very early control of the p50 transcription factor and provide a new perspective on Rel protein assembly.	transcription
55988	1	335298	7	NULL	NULL	0	NULL	p105 inhibitor			gains early control of					p50 transcription factor					NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_40	10970863	These results highlight a mechanism by which the p105 inhibitor gains very early control of the p50 transcription factor and provide a new perspective on Rel protein assembly.	transcription
55989	2	335298	7	NULL	NULL	0	NULL	statement 1			provide					Rel protein assembly		new prespective on			NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_40	10970863	These results highlight a mechanism by which the p105 inhibitor gains very early control of the p50 transcription factor and provide a new perspective on Rel protein assembly.	transcription
54881	1	335299	5	NULL	NULL	0	NULL	p105			is processed to					p50					NULL		0	NULL	NULL	NULL	gw60_embo_19_11_2580_s_49	10835356	Here we show that IkappaKbeta-mediated phosphorylation at the C-terminal domain results in accelerated processing of p105 to p50, a process that is mediated by the SCFbeta-TrCP E3.	transcription
54882	2	335299	5	NULL	NULL	0	NULL	IkappaKbeta			mediates					p105		phosphorylation of	C-terminus		NULL		0	NULL	NULL	NULL	gw60_embo_19_11_2580_s_49	10835356	Here we show that IkappaKbeta-mediated phosphorylation at the C-terminal domain results in accelerated processing of p105 to p50, a process that is mediated by the SCFbeta-TrCP E3.	transcription
54883	3	335299	5	NULL	NULL	0	NULL	statement 2			results in					statement 1		accelerated			NULL		0	NULL	NULL	NULL	gw60_embo_19_11_2580_s_49	10835356	Here we show that IkappaKbeta-mediated phosphorylation at the C-terminal domain results in accelerated processing of p105 to p50, a process that is mediated by the SCFbeta-TrCP E3.	transcription
54884	4	335299	5	NULL	NULL	0	NULL	SCFbeta-TrCP E3			mediates					statement 1		accelerated			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_11_2580_s_49	10835356	Here we show that IkappaKbeta-mediated phosphorylation at the C-terminal domain results in accelerated processing of p105 to p50, a process that is mediated by the SCFbeta-TrCP E3.	transcription
55990	1	335299	7	NULL	NULL	0	NULL	 IkappaKbeta			mediates							phosphorylation at	C-terminal domain		NULL		0	NULL	NULL	NULL	gw60_embo_19_11_2580_s_49	10835356	Here we show that IkappaKbeta-mediated phosphorylation at the C-terminal domain results in accelerated processing of p105 to p50, a process that is mediated by the SCFbeta-TrCP E3.	transcription
55991	2	335299	7	NULL	NULL	0	NULL	p105			processed to					p50					NULL		0	NULL	NULL	NULL	gw60_embo_19_11_2580_s_49	10835356	Here we show that IkappaKbeta-mediated phosphorylation at the C-terminal domain results in accelerated processing of p105 to p50, a process that is mediated by the SCFbeta-TrCP E3.	transcription
55992	3	335299	7	NULL	NULL	0	NULL	statement 1			accelerates					statement 2					NULL		0	NULL	NULL	NULL	gw60_embo_19_11_2580_s_49	10835356	Here we show that IkappaKbeta-mediated phosphorylation at the C-terminal domain results in accelerated processing of p105 to p50, a process that is mediated by the SCFbeta-TrCP E3.	transcription
55993	4	335299	7	NULL	NULL	0	NULL	SCFbeta-TrCP E3			mediates					statement 3					NULL		0	NULL	NULL	NULL	gw60_embo_19_11_2580_s_49	10835356	Here we show that IkappaKbeta-mediated phosphorylation at the C-terminal domain results in accelerated processing of p105 to p50, a process that is mediated by the SCFbeta-TrCP E3.	transcription
54885	1	335300	5	NULL	NULL	0	NULL	p105			is targeted of		may	glycine-rich region		endoprotease					NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_31	10469655	C-terminal to the p50 moiety, p105 contains a glycine-rich region which is required for processing in mammalian cells and may be the target of an endoprotease (Lin and Ghosh, 1996  ).	transcription
55994	1	335300	7	NULL	NULL	0	NULL	p105			contains								glycine-rich region		NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_31	10469655	C-terminal to the p50 moiety, p105 contains a glycine-rich region which is required for processing in mammalian cells and may be the target of an endoprotease (Lin and Ghosh, 1996  ).	transcription
55995	2	335300	7	NULL	NULL	0	NULL	statement 1			is required for					mammalian cells		processing in			NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_31	10469655	C-terminal to the p50 moiety, p105 contains a glycine-rich region which is required for processing in mammalian cells and may be the target of an endoprotease (Lin and Ghosh, 1996  ).	transcription
55996	3	335300	7	NULL	NULL	0	NULL	statement 1			be target for		may			endoprotease					NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_31	10469655	C-terminal to the p50 moiety, p105 contains a glycine-rich region which is required for processing in mammalian cells and may be the target of an endoprotease (Lin and Ghosh, 1996  ).	transcription
54886	1	335301	5	NULL	NULL	0	NULL	BCL-3			is a type of					oncoprotein					NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_19	9529257	Additionally, the candidate oncoprotein BCL-3 induces p50 homodimers from cytosolic p105/p50 complexes without  enhancing the processing of p105 (Watanabe et al., 1997   ).	transcription
54887	2	335301	5	NULL	NULL	0	NULL	p50 homodimers			formed from					p105/p50 complexes		cytosolic			NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_19	9529257	Additionally, the candidate oncoprotein BCL-3 induces p50 homodimers from cytosolic p105/p50 complexes without  enhancing the processing of p105 (Watanabe et al., 1997   ).	transcription
54888	3	335301	5	NULL	NULL	0	NULL	statement 2			does not enhance					p105		processing of			NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_19	9529257	Additionally, the candidate oncoprotein BCL-3 induces p50 homodimers from cytosolic p105/p50 complexes without  enhancing the processing of p105 (Watanabe et al., 1997   ).	transcription
54889	4	335301	5	NULL	NULL	0	NULL	BCL-3			induces					statement 3					NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_19	9529257	Additionally, the candidate oncoprotein BCL-3 induces p50 homodimers from cytosolic p105/p50 complexes without  enhancing the processing of p105 (Watanabe et al., 1997   ).	transcription
55997	1	335301	7	NULL	NULL	0	NULL	p50 homodimers			obtained from					p105/p50 complexes		cytosolic			NULL		NULL	NULL	NULL	NULL	gw60_cell_92_6_819_s_19	9529257	Additionally, the candidate oncoprotein BCL-3 induces p50 homodimers from cytosolic p105/p50 complexes without  enhancing the processing of p105 (Watanabe et al., 1997   ).	transcription
55998	2	335301	7	NULL	NULL	0	NULL	BCL-3 			induce					statement 1					NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_19	9529257	Additionally, the candidate oncoprotein BCL-3 induces p50 homodimers from cytosolic p105/p50 complexes without  enhancing the processing of p105 (Watanabe et al., 1997   ).	transcription
55999	3	335301	7	NULL	NULL	0	NULL	BCL-3 			does not enhance					p105		processing of			NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_19	9529257	Additionally, the candidate oncoprotein BCL-3 induces p50 homodimers from cytosolic p105/p50 complexes without  enhancing the processing of p105 (Watanabe et al., 1997   ).	transcription
56000	4	335301	7	NULL	NULL	0	NULL	BCL-3 			is a type of					oncoprotein					NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_19	9529257	Additionally, the candidate oncoprotein BCL-3 induces p50 homodimers from cytosolic p105/p50 complexes without  enhancing the processing of p105 (Watanabe et al., 1997   ).	transcription
54890	1	335302	5	NULL	NULL	0	NULL	Ang II			effect		delayed			NF-kappaB1		processing of			NULL	VSMCs	0	NULL	NULL	NULL	gw60_circulationres_84_6_695_s_253	10189357	Our data also implicate a delayed effect of Ang II on NF-kappaB1 processing in VSMCs. NF-kappaB1 p50 is the NH2-terminal DNA-binding product of p105 precursor processing.	transcription
54891	2	335302	5	NULL	NULL	0	NULL	NF-kappaB1 p50			is a product of					p105 precursor		processing of			NULL		0	NULL	NULL	NULL	gw60_circulationres_84_6_695_s_253	10189357	Our data also implicate a delayed effect of Ang II on NF-kappaB1 processing in VSMCs. NF-kappaB1 p50 is the NH2-terminal DNA-binding product of p105 precursor processing.	transcription
56001	1	335302	7	NULL	NULL	0	NULL	NF-kappaB1 p50			is a type of								NH2-terminal DNA-binding product		NULL		0	NULL	NULL	NULL	gw60_circulationres_84_6_695_s_253	10189357	Our data also implicate a delayed effect of Ang II on NF-kappaB1 processing in VSMCs. NF-kappaB1 p50 is the NH2-terminal DNA-binding product of p105 precursor processing.	transcription
56002	2	335302	7	NULL	NULL	0	NULL	statement 1			is obtained from					p105 precursor		processing of			NULL		0	NULL	NULL	NULL	gw60_circulationres_84_6_695_s_253	10189357	Our data also implicate a delayed effect of Ang II on NF-kappaB1 processing in VSMCs. NF-kappaB1 p50 is the NH2-terminal DNA-binding product of p105 precursor processing.	transcription
54892	1	335303	5	NULL	NULL	0	NULL	TPL-2			co-immunoprecipitates with		specifically			p50					NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_109	9950430	As TPL-2 specifically co-immunoprecipitates with p50, Rel-A and c-Rel ( Fig.3a), it may regulate proteolysis of all of the major p105 complexes present in cells 6, 7.	transcription
54893	2	335303	5	NULL	NULL	0	NULL	TPL-2			co-immunoprecipitates with		specifically			Rel-A					NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_109	9950430	As TPL-2 specifically co-immunoprecipitates with p50, Rel-A and c-Rel ( Fig.3a), it may regulate proteolysis of all of the major p105 complexes present in cells 6, 7.	transcription
54894	3	335303	5	NULL	NULL	0	NULL	TPL-2			co-immunoprecipitates with		specifically			c-Rel					NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_109	9950430	As TPL-2 specifically co-immunoprecipitates with p50, Rel-A and c-Rel ( Fig.3a), it may regulate proteolysis of all of the major p105 complexes present in cells 6, 7.	transcription
54895	4	335303	5	NULL	NULL	0	NULL	TPL-2			regulates		may			p105 complexes		proteolysis of major 			NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_109	9950430	As TPL-2 specifically co-immunoprecipitates with p50, Rel-A and c-Rel ( Fig.3a), it may regulate proteolysis of all of the major p105 complexes present in cells 6, 7.	transcription
56003	1	335303	7	NULL	NULL	0	NULL	TPL-2			bind		specifically			p50					NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_109	9950430	As TPL-2 specifically co-immunoprecipitates with p50, Rel-A and c-Rel ( Fig.3a), it may regulate proteolysis of all of the major p105 complexes present in cells 6, 7.	transcription
56004	2	335303	7	NULL	NULL	0	NULL	TPL-2			bind		specifically			Rel-A					NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_109	9950430	As TPL-2 specifically co-immunoprecipitates with p50, Rel-A and c-Rel ( Fig.3a), it may regulate proteolysis of all of the major p105 complexes present in cells 6, 7.	transcription
56005	3	335303	7	NULL	NULL	0	NULL	TPL-2 			bind		specifically			c-Rel					NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_109	9950430	As TPL-2 specifically co-immunoprecipitates with p50, Rel-A and c-Rel ( Fig.3a), it may regulate proteolysis of all of the major p105 complexes present in cells 6, 7.	transcription
56006	4	335303	7	NULL	NULL	0	NULL	statement 1			regulate		may			p105 complex		proteolysis of			NULL	cells	0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_109	9950430	As TPL-2 specifically co-immunoprecipitates with p50, Rel-A and c-Rel ( Fig.3a), it may regulate proteolysis of all of the major p105 complexes present in cells 6, 7.	transcription
56007	5	335303	7	NULL	NULL	0	NULL	statement 2			regulate		may			p105 complex		proteolysis of			NULL	cells	0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_109	9950430	As TPL-2 specifically co-immunoprecipitates with p50, Rel-A and c-Rel ( Fig.3a), it may regulate proteolysis of all of the major p105 complexes present in cells 6, 7.	transcription
56008	6	335303	7	NULL	NULL	0	NULL	statement 3			regulate		may			p105 complex		proteolysis of			NULL	cells	0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_109	9950430	As TPL-2 specifically co-immunoprecipitates with p50, Rel-A and c-Rel ( Fig.3a), it may regulate proteolysis of all of the major p105 complexes present in cells 6, 7.	transcription
54896	1	335304	5	NULL	NULL	0	NULL	p105			interacts with			C-terminal region		p50			nuclear localization signal		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_512_s_641	9418898	Interaction of the C-terminal region of p105 with the nuclear localization signal of p50 is required for inhibition of NF-kappa B DNA binding activity.	transcription
54897	2	335304	5	NULL	NULL	0	NULL	NF-kappa B			bind					DNA					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_512_s_641	9418898	Interaction of the C-terminal region of p105 with the nuclear localization signal of p50 is required for inhibition of NF-kappa B DNA binding activity.	transcription
54898	3	335304	5	NULL	NULL	0	NULL	statement 1			is required for					statement 2		inhibition of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_512_s_641	9418898	Interaction of the C-terminal region of p105 with the nuclear localization signal of p50 is required for inhibition of NF-kappa B DNA binding activity.	transcription
56009	1	335304	7	NULL	NULL	0	NULL	p105 			interacts with			C-terminal region		p50			nuclear localization signal		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_512_s_641	9418898	Interaction of the C-terminal region of p105 with the nuclear localization signal of p50 is required for inhibition of NF-kappa B DNA binding activity.	transcription
56010	2	335304	7	NULL	NULL	0	NULL	NF-kappa B 			bind					DNA					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_512_s_641	9418898	Interaction of the C-terminal region of p105 with the nuclear localization signal of p50 is required for inhibition of NF-kappa B DNA binding activity.	transcription
56011	3	335304	7	NULL	NULL	0	NULL	statement 1			is required for					statement 2		inhibition of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_512_s_641	9418898	Interaction of the C-terminal region of p105 with the nuclear localization signal of p50 is required for inhibition of NF-kappa B DNA binding activity.	transcription
54899	1	335305	5	NULL	NULL	0	NULL	LPS			is					lipopolysaccharide					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_12	11158290	In line with this and as a physiologically relevant model, lipopolysaccharide (LPS) induced degradation of endogenous p105 and p50 homodimer formation, but not processing in pre-B cells.	transcription
54900	2	335305	5	NULL	NULL	0	NULL	LPS			induces					p105		degradation of;;endogenous			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_12	11158290	In line with this and as a physiologically relevant model, lipopolysaccharide (LPS) induced degradation of endogenous p105 and p50 homodimer formation, but not processing in pre-B cells.	transcription
54901	3	335305	5	NULL	NULL	0	NULL	LPS			induces					p50 homodimer		formation of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_12	11158290	In line with this and as a physiologically relevant model, lipopolysaccharide (LPS) induced degradation of endogenous p105 and p50 homodimer formation, but not processing in pre-B cells.	transcription
56012	1	335305	7	NULL	NULL	0	NULL	p105		endogenous	homodimerize with					p105		endogenous			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_12	11158290	In line with this and as a physiologically relevant model, lipopolysaccharide (LPS) induced degradation of endogenous p105 and p50 homodimer formation, but not processing in pre-B cells.	transcription
56013	2	335305	7	NULL	NULL	0	NULL	p50		endogenous	homodimerize with					p50		endogenous			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_12	11158290	In line with this and as a physiologically relevant model, lipopolysaccharide (LPS) induced degradation of endogenous p105 and p50 homodimer formation, but not processing in pre-B cells.	transcription
56014	3	335305	7	NULL	NULL	0	NULL	LPS			induce					statement 1		degradation of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_12	11158290	In line with this and as a physiologically relevant model, lipopolysaccharide (LPS) induced degradation of endogenous p105 and p50 homodimer formation, but not processing in pre-B cells.	transcription
56015	4	335305	7	NULL	NULL	0	NULL	LPS			induce					statement 2		degradation of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_12	11158290	In line with this and as a physiologically relevant model, lipopolysaccharide (LPS) induced degradation of endogenous p105 and p50 homodimer formation, but not processing in pre-B cells.	transcription
56016	5	335305	7	NULL	NULL	0	NULL	LPS			is					lipopolysaccharide					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_12	11158290	In line with this and as a physiologically relevant model, lipopolysaccharide (LPS) induced degradation of endogenous p105 and p50 homodimer formation, but not processing in pre-B cells.	transcription
56017	6	335305	7	NULL	NULL	0	NULL	LPS			does not induce					p105		processing of			NULL	pre-B cells	0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_12	11158290	In line with this and as a physiologically relevant model, lipopolysaccharide (LPS) induced degradation of endogenous p105 and p50 homodimer formation, but not processing in pre-B cells.	transcription
56018	7	335305	7	NULL	NULL	0	NULL	LPS			does not induce					p50		processing of			NULL	pre-B cells	0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_12	11158290	In line with this and as a physiologically relevant model, lipopolysaccharide (LPS) induced degradation of endogenous p105 and p50 homodimer formation, but not processing in pre-B cells.	transcription
54902	1	335306	5	NULL	NULL	0	NULL	IKK complex		functional;;endogenous	contains					IKKgamma					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_257	11158290	Taken together, these data demonstrate that a functional endogenous IKK complex containing IKKgamma is required for LPS-induced p105 degradation and p50 release.	transcription
54903	2	335306	5	NULL	NULL	0	NULL	LPS			induces					p105		degradation of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_257	11158290	Taken together, these data demonstrate that a functional endogenous IKK complex containing IKKgamma is required for LPS-induced p105 degradation and p50 release.	transcription
54904	3	335306	5	NULL	NULL	0	NULL	statement 2			releases					p50					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_257	11158290	Taken together, these data demonstrate that a functional endogenous IKK complex containing IKKgamma is required for LPS-induced p105 degradation and p50 release.	transcription
54905	4	335306	5	NULL	NULL	0	NULL	statement 1			is required for					statement 2					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_257	11158290	Taken together, these data demonstrate that a functional endogenous IKK complex containing IKKgamma is required for LPS-induced p105 degradation and p50 release.	transcription
54906	5	335306	5	NULL	NULL	0	NULL	statement 1			is required for					statement 3					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_257	11158290	Taken together, these data demonstrate that a functional endogenous IKK complex containing IKKgamma is required for LPS-induced p105 degradation and p50 release.	transcription
56019	1	335306	7	NULL	NULL	0	NULL	LPS			induce					p105		degradation of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_257	11158290	Taken together, these data demonstrate that a functional endogenous IKK complex containing IKKgamma is required for LPS-induced p105 degradation and p50 release.	transcription
56020	2	335306	7	NULL	NULL	0	NULL	LPS			induce					p50		release of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_257	11158290	Taken together, these data demonstrate that a functional endogenous IKK complex containing IKKgamma is required for LPS-induced p105 degradation and p50 release.	transcription
56021	3	335306	7	NULL	NULL	0	NULL	IKK complex		 functional;;endogenous	contains					IKKgamma					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_257	11158290	Taken together, these data demonstrate that a functional endogenous IKK complex containing IKKgamma is required for LPS-induced p105 degradation and p50 release.	transcription
56022	4	335306	7	NULL	NULL	0	NULL	statement 3			is required for					statement 1					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_257	11158290	Taken together, these data demonstrate that a functional endogenous IKK complex containing IKKgamma is required for LPS-induced p105 degradation and p50 release.	transcription
56023	5	335306	7	NULL	NULL	0	NULL	statement 3			is required for					statement 2					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_257	11158290	Taken together, these data demonstrate that a functional endogenous IKK complex containing IKKgamma is required for LPS-induced p105 degradation and p50 release.	transcription
54907	1	335307	5	NULL	NULL	0	NULL	p50		overexpressed	does not affect					p105- Tth111		processing of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_180	11350967	As can be seen in Fig.  5 A, overexpressed p50 does not affect processing of p105- Tth111 (11%; compare  lanes 1 and  2 with  lanes 3 and  4).	transcription
56024	1	335307	7	NULL	NULL	0	NULL	 p50		overexpressed	does not affect					p105- Tth111		processing of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_180	11350967	As can be seen in Fig.  5 A, overexpressed p50 does not affect processing of p105- Tth111 (11%; compare  lanes 1 and  2 with  lanes 3 and  4).	transcription
54908	1	335308	5	NULL	NULL	0	NULL	IKK			mediates					p105		degradation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_238	11350967	Heissmeyer and colleagues ( 15) have shown that IKK-mediated degradation of p105 releases docked p50 that interacts with Bcl-3 to generate the trimeric p50.p50.Bcl-3 active transcription factor.	transcription
54909	2	335308	5	NULL	NULL	0	NULL	statement 1			releases					p50		docked			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_238	11350967	Heissmeyer and colleagues ( 15) have shown that IKK-mediated degradation of p105 releases docked p50 that interacts with Bcl-3 to generate the trimeric p50.p50.Bcl-3 active transcription factor.	transcription
54910	3	335308	5	NULL	NULL	0	NULL	p50			interacts with					Bcl-3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_238	11350967	Heissmeyer and colleagues ( 15) have shown that IKK-mediated degradation of p105 releases docked p50 that interacts with Bcl-3 to generate the trimeric p50.p50.Bcl-3 active transcription factor.	transcription
54911	4	335308	5	NULL	NULL	0	NULL	statement 3			generates					p50.p50.Bcl-3 timer					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_238	11350967	Heissmeyer and colleagues ( 15) have shown that IKK-mediated degradation of p105 releases docked p50 that interacts with Bcl-3 to generate the trimeric p50.p50.Bcl-3 active transcription factor.	transcription
54912	5	335308	5	NULL	NULL	0	NULL	p50.p50.Bcl-3 trimer			is a type of					active transcription factor					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_238	11350967	Heissmeyer and colleagues ( 15) have shown that IKK-mediated degradation of p105 releases docked p50 that interacts with Bcl-3 to generate the trimeric p50.p50.Bcl-3 active transcription factor.	transcription
56025	1	335308	7	NULL	NULL	0	NULL	IKK			mediate					p105		degradation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_238	11350967	Heissmeyer and colleagues ( 15) have shown that IKK-mediated degradation of p105 releases docked p50 that interacts with Bcl-3 to generate the trimeric p50.p50.Bcl-3 active transcription factor.	transcription
56026	2	335308	7	NULL	NULL	0	NULL	statement 1			release					p50		docked			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_238	11350967	Heissmeyer and colleagues ( 15) have shown that IKK-mediated degradation of p105 releases docked p50 that interacts with Bcl-3 to generate the trimeric p50.p50.Bcl-3 active transcription factor.	transcription
56027	3	335308	7	NULL	NULL	0	NULL	p50			interacts with					Bcl-3 					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_238	11350967	Heissmeyer and colleagues ( 15) have shown that IKK-mediated degradation of p105 releases docked p50 that interacts with Bcl-3 to generate the trimeric p50.p50.Bcl-3 active transcription factor.	transcription
56028	4	335308	7	NULL	NULL	0	NULL	statement 3			generate					p50.p50.Bcl-3		trimeric			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_238	11350967	Heissmeyer and colleagues ( 15) have shown that IKK-mediated degradation of p105 releases docked p50 that interacts with Bcl-3 to generate the trimeric p50.p50.Bcl-3 active transcription factor.	transcription
56029	5	335308	7	NULL	NULL	0	NULL	p50.p50.Bcl-3			is a type of					active transcription factor					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_238	11350967	Heissmeyer and colleagues ( 15) have shown that IKK-mediated degradation of p105 releases docked p50 that interacts with Bcl-3 to generate the trimeric p50.p50.Bcl-3 active transcription factor.	transcription
54913	1	335309	5	NULL	NULL	0	NULL	p105		transcription of	is induced by					IKK					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_302	11350967	The researchers argue, although they do not provide direct experimental evidence, that the increased amount of p50 observed under these conditions is attributed to increased transcription of p105 induced by IKK.	transcription
54914	1	335309	5	NULL	NULL	0	NULL	p105		transcription of	is induced by					IKK					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_302	11350967	The researchers argue, although they do not provide direct experimental evidence, that the increased amount of p50 observed under these conditions is attributed to increased transcription of p105 induced by IKK.	transcription
54915	2	335309	5	NULL	NULL	0	NULL	statement 1		increased	leads to					p50		increased			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_302	11350967	The researchers argue, although they do not provide direct experimental evidence, that the increased amount of p50 observed under these conditions is attributed to increased transcription of p105 induced by IKK.	transcription
56030	1	335309	7	NULL	NULL	0	NULL	 IKK			induce					p105		increased transcription of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_302	11350967	The researchers argue, although they do not provide direct experimental evidence, that the increased amount of p50 observed under these conditions is attributed to increased transcription of p105 induced by IKK.	transcription
54916	1	335310	5	NULL	NULL	0	NULL	proteasome			activates		proteolytically			NFkappaB					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_19_16802_s_218	12615917	For example, the first step in the proteolytic activation of NFkappaB from its precursor protein p105 to yield p50 is catalyzed by the proteasome ( 37,  46).	transcription
54917	2	335310	5	NULL	NULL	0	NULL	p105 precursor protein			yields					p50					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_19_16802_s_218	12615917	For example, the first step in the proteolytic activation of NFkappaB from its precursor protein p105 to yield p50 is catalyzed by the proteasome ( 37,  46).	transcription
54918	3	335310	5	NULL	NULL	0	NULL	statement 1			leads to					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_19_16802_s_218	12615917	For example, the first step in the proteolytic activation of NFkappaB from its precursor protein p105 to yield p50 is catalyzed by the proteasome ( 37,  46).	transcription
56031	2	335310	7	NULL	NULL	0	NULL	statement 1			is obtained from					p105					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_19_16802_s_218	12615917	For example, the first step in the proteolytic activation of NFkappaB from its precursor protein p105 to yield p50 is catalyzed by the proteasome ( 37,  46).	transcription
56032	1	335310	7	NULL	NULL	0	NULL	proteasome 			catalyze					NFkappaB		proteolytic activation of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_19_16802_s_218	12615917	For example, the first step in the proteolytic activation of NFkappaB from its precursor protein p105 to yield p50 is catalyzed by the proteasome ( 37,  46).	transcription
56033	4	335310	7	NULL	NULL	0	NULL	p105			is a precursor of					NFkappaB					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_19_16802_s_218	12615917	For example, the first step in the proteolytic activation of NFkappaB from its precursor protein p105 to yield p50 is catalyzed by the proteasome ( 37,  46).	transcription
56034	3	335310	7	NULL	NULL	0	NULL	statement 1			yield					p50					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_19_16802_s_218	12615917	For example, the first step in the proteolytic activation of NFkappaB from its precursor protein p105 to yield p50 is catalyzed by the proteasome ( 37,  46).	transcription
54919	1	335311	5	NULL	NULL	0	NULL	NF-kappaB inducers		treatment	results in					p105		phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_3_1409_s_25	9430676	Analogous to the situation for IkappaB-alpha, treatment of cells with inducers of NF-kappaB results in the phosphorylation of p105 ( 23-26), and an increase in the level of p50 is observed ( 27-29).	transcription
54920	2	335311	5	NULL	NULL	0	NULL	statement 1			leads to					p50		increase in level of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_3_1409_s_25	9430676	Analogous to the situation for IkappaB-alpha, treatment of cells with inducers of NF-kappaB results in the phosphorylation of p105 ( 23-26), and an increase in the level of p50 is observed ( 27-29).	transcription
56913	1	335311	7	NULL	NULL	0	NULL	 NF-kappaB 		inducers of	result in					p105		phosphorylation of			NULL	cells	0	NULL	NULL	NULL	gw60_jbiolchem_273_3_1409_s_25	9430676	Analogous to the situation for IkappaB-alpha, treatment of cells with inducers of NF-kappaB results in the phosphorylation of p105 ( 23-26), and an increase in the level of p50 is observed ( 27-29).	transcription
56914	2	335311	7	NULL	NULL	0	NULL	 NF-kappaB 		inducers of	increase					p50		level of			NULL	cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_3_1409_s_25	9430676	Analogous to the situation for IkappaB-alpha, treatment of cells with inducers of NF-kappaB results in the phosphorylation of p105 ( 23-26), and an increase in the level of p50 is observed ( 27-29).	transcription
54921	1	335312	5	NULL	NULL	0	NULL	p105			is cleaved to					p50					NULL		0	NULL	NULL	NULL	gw60_science_295_5556_813_s_172	11823631	Thus, two proteolytic events--the cleavage of p105 to p50 and  the destruction of IkappaB governed by serine  phosphorylation--are required to produce the proteins and then activate them.	transcription
54922	2	335312	5	NULL	NULL	0	NULL	IkappaB		destruction of	is governed by					serine		phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_science_295_5556_813_s_172	11823631	Thus, two proteolytic events--the cleavage of p105 to p50 and  the destruction of IkappaB governed by serine  phosphorylation--are required to produce the proteins and then activate them.	transcription
56915	1	335312	7	NULL	NULL	0	NULL	 p105			cleaved to					p50					NULL		0	NULL	NULL	NULL	gw60_science_295_5556_813_s_172	11823631	Thus, two proteolytic events--the cleavage of p105 to p50 and  the destruction of IkappaB governed by serine  phosphorylation--are required to produce the proteins and then activate them.	transcription
56916	2	335312	7	NULL	NULL	0	NULL	serine 		phosphorylation of	governs					statement 1					NULL		0	NULL	NULL	NULL	gw60_science_295_5556_813_s_172	11823631	Thus, two proteolytic events--the cleavage of p105 to p50 and  the destruction of IkappaB governed by serine  phosphorylation--are required to produce the proteins and then activate them.	transcription
56917	3	335312	7	NULL	NULL	0	NULL	serine		phosphorylation of	governs					IkappaB		destruction of			NULL		0	NULL	NULL	NULL	gw60_science_295_5556_813_s_172	11823631	Thus, two proteolytic events--the cleavage of p105 to p50 and  the destruction of IkappaB governed by serine  phosphorylation--are required to produce the proteins and then activate them.	transcription
54923	1	335313	5	NULL	NULL	0	NULL	p105sr			inhibits		efficiently			NF-kappaB		activity of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_36_26041_s_113	16835236	Consequently, p105sr efficiently inhibits all NF-kappaB activities, including p50 homodimers ( ).	transcription
54924	2	335313	5	NULL	NULL	0	NULL	p105sr			inhibits		efficiently			p50 homodimer					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_36_26041_s_113	16835236	Consequently, p105sr efficiently inhibits all NF-kappaB activities, including p50 homodimers ( ).	transcription
56918	1	335313	7	NULL	NULL	0	NULL	 p105sr			inhibits		efficiently			NF-kappaB 		all activities of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_36_26041_s_113	16835236	Consequently, p105sr efficiently inhibits all NF-kappaB activities, including p50 homodimers ( ).	transcription
56919	2	335313	7	NULL	NULL	0	NULL	NF-kappaB			include					p50 homodimers					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_36_26041_s_113	16835236	Consequently, p105sr efficiently inhibits all NF-kappaB activities, including p50 homodimers ( ).	transcription
56931	1	335314	7	NULL	NULL	0	NULL	p50			generated by					proteasome					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_12_8646_s_209	10567588	To investigate whether the reduced expression of p50 in NOD mouse spleen cells is attributable to defective p50 generation by the proteasome, we examined p50 generation by cytosolic extracts by using an in vitro assay in which 35S-labeled recombinant p105, or the truncated version, p60Tth, was used as the substrate ( 19,  61).	transcription
56932	2	335314	7	NULL	NULL	0	NULL	p50		reduced expression of	is attributed to					statement 1		defective			NULL	NOD mouse spleen cells	0	NULL	NULL	NULL	gw60_molcellbiol_19_12_8646_s_209	10567588	To investigate whether the reduced expression of p50 in NOD mouse spleen cells is attributable to defective p50 generation by the proteasome, we examined p50 generation by cytosolic extracts by using an in vitro assay in which 35S-labeled recombinant p105, or the truncated version, p60Tth, was used as the substrate ( 19,  61).	transcription
54925	1	335315	5	NULL	NULL	0	NULL	p105 protein		post-translational modifications of	leads to					p50		increase in level of			NULL	tolerant T cells	0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8460_s_30	14668329	Because transcriptional induction of the precursor protein p105 did not differ between tolerant and activated T cells, our data suggest that the overall increased levels of p50 in tolerant T cells may be due to post-translational modifications of the p105 protein.	transcription
56933	1	335315	7	NULL	NULL	0	NULL	p50		increased levels of;;tolerant T cells	due to					p105 protein		 post-translational modifications of 			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_8460_s_30	14668329	Because transcriptional induction of the precursor protein p105 did not differ between tolerant and activated T cells, our data suggest that the overall increased levels of p50 in tolerant T cells may be due to post-translational modifications of the p105 protein.	transcription
56934	2	335315	7	NULL	NULL	0	NULL	p105		transcriptional induction of ;;tolerant T cells	does not differ  from					p105		transcriptional induction of ;;activated T cells			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_8460_s_30	14668329	Because transcriptional induction of the precursor protein p105 did not differ between tolerant and activated T cells, our data suggest that the overall increased levels of p50 in tolerant T cells may be due to post-translational modifications of the p105 protein.	transcription
56935	3	335315	7	NULL	NULL	0	NULL	p105			is a type of					precursor protein					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8460_s_30	14668329	Because transcriptional induction of the precursor protein p105 did not differ between tolerant and activated T cells, our data suggest that the overall increased levels of p50 in tolerant T cells may be due to post-translational modifications of the p105 protein.	transcription
54934	1	335316	5	NULL	NULL	0	NULL	p50			constitutes					p105			NH2-terminus		NULL		0	NULL	NULL	NULL	gw70_science_299_5605_408_s_8	12481023	Because p50 constitutes the NH2-terminus of p105 and the COOH-terminus is presumably blocked by the ribosome, the proteasome must either wait for release of nascent p105 from the ribosome or activate another protease that catalyzes the initial endoproteolytic step, as in the proteasome-dependent activation of Esp1 protease during sister chromatid exchange ( 9).	transcription
54935	2	335316	5	NULL	NULL	0	NULL	p105			is blocked by		presumably	COOH-terminus		ribosome					NULL		0	NULL	NULL	NULL	gw70_science_299_5605_408_s_8	12481023	Because p50 constitutes the NH2-terminus of p105 and the COOH-terminus is presumably blocked by the ribosome, the proteasome must either wait for release of nascent p105 from the ribosome or activate another protease that catalyzes the initial endoproteolytic step, as in the proteasome-dependent activation of Esp1 protease during sister chromatid exchange ( 9).	transcription
54936	3	335316	5	NULL	NULL	0	NULL	p105		nascent	is released from					ribosome					NULL		NULL	NULL	NULL	NULL	gw70_science_299_5605_408_s_8	12481023	Because p50 constitutes the NH2-terminus of p105 and the COOH-terminus is presumably blocked by the ribosome, the proteasome must either wait for release of nascent p105 from the ribosome or activate another protease that catalyzes the initial endoproteolytic step, as in the proteasome-dependent activation of Esp1 protease during sister chromatid exchange ( 9).	transcription
54937	4	335316	5	NULL	NULL	0	NULL	proteasome			waits for		may			statement 3					NULL		0	NULL	NULL	NULL	gw70_science_299_5605_408_s_8	12481023	Because p50 constitutes the NH2-terminus of p105 and the COOH-terminus is presumably blocked by the ribosome, the proteasome must either wait for release of nascent p105 from the ribosome or activate another protease that catalyzes the initial endoproteolytic step, as in the proteasome-dependent activation of Esp1 protease during sister chromatid exchange ( 9).	transcription
54938	5	335316	5	NULL	NULL	0	NULL	proteasome			activates		may			protease					NULL		0	NULL	NULL	NULL	gw70_science_299_5605_408_s_8	12481023	Because p50 constitutes the NH2-terminus of p105 and the COOH-terminus is presumably blocked by the ribosome, the proteasome must either wait for release of nascent p105 from the ribosome or activate another protease that catalyzes the initial endoproteolytic step, as in the proteasome-dependent activation of Esp1 protease during sister chromatid exchange ( 9).	transcription
54939	6	335316	5	NULL	NULL	0	NULL	statement 5			catalyze					endoproteolytic step		initial			NULL		0	NULL	NULL	NULL	gw70_science_299_5605_408_s_8	12481023	Because p50 constitutes the NH2-terminus of p105 and the COOH-terminus is presumably blocked by the ribosome, the proteasome must either wait for release of nascent p105 from the ribosome or activate another protease that catalyzes the initial endoproteolytic step, as in the proteasome-dependent activation of Esp1 protease during sister chromatid exchange ( 9).	transcription
54940	7	335316	5	NULL	NULL	0	NULL	statement 4			is an alternative to					statement 5					NULL		0	NULL	NULL	NULL	gw70_science_299_5605_408_s_8	12481023	Because p50 constitutes the NH2-terminus of p105 and the COOH-terminus is presumably blocked by the ribosome, the proteasome must either wait for release of nascent p105 from the ribosome or activate another protease that catalyzes the initial endoproteolytic step, as in the proteasome-dependent activation of Esp1 protease during sister chromatid exchange ( 9).	transcription
54941	8	335316	5	NULL	NULL	0	NULL	Esp1			is a type of					protease					NULL		0	NULL	NULL	NULL	gw70_science_299_5605_408_s_8	12481023	Because p50 constitutes the NH2-terminus of p105 and the COOH-terminus is presumably blocked by the ribosome, the proteasome must either wait for release of nascent p105 from the ribosome or activate another protease that catalyzes the initial endoproteolytic step, as in the proteasome-dependent activation of Esp1 protease during sister chromatid exchange ( 9).	transcription
54942	9	335316	5	NULL	NULL	0	NULL	Esp1		activation of	is dependent on					proteasome					NULL		0	NULL	NULL	NULL	gw70_science_299_5605_408_s_8	12481023	Because p50 constitutes the NH2-terminus of p105 and the COOH-terminus is presumably blocked by the ribosome, the proteasome must either wait for release of nascent p105 from the ribosome or activate another protease that catalyzes the initial endoproteolytic step, as in the proteasome-dependent activation of Esp1 protease during sister chromatid exchange ( 9).	transcription
54943	10	335316	5	NULL	NULL	0	NULL	statement 9			occurs during					sister chromatid exchange					NULL		0	NULL	NULL	NULL	gw70_science_299_5605_408_s_8	12481023	Because p50 constitutes the NH2-terminus of p105 and the COOH-terminus is presumably blocked by the ribosome, the proteasome must either wait for release of nascent p105 from the ribosome or activate another protease that catalyzes the initial endoproteolytic step, as in the proteasome-dependent activation of Esp1 protease during sister chromatid exchange ( 9).	transcription
56936	1	335316	7	NULL	NULL	0	NULL	p50			constitute					p105			NH2-terminus		NULL		0	NULL	NULL	NULL	gw70_science_299_5605_408_s_8	12481023	Because p50 constitutes the NH2-terminus of p105 and the COOH-terminus is presumably blocked by the ribosome, the proteasome must either wait for release of nascent p105 from the ribosome or activate another protease that catalyzes the initial endoproteolytic step, as in the proteasome-dependent activation of Esp1 protease during sister chromatid exchange ( 9).	transcription
56937	2	335316	7	NULL	NULL	0	NULL	p105			blocked by		presumably	COOH-terminus		ribosome					NULL		0	NULL	NULL	NULL	gw70_science_299_5605_408_s_8	12481023	Because p50 constitutes the NH2-terminus of p105 and the COOH-terminus is presumably blocked by the ribosome, the proteasome must either wait for release of nascent p105 from the ribosome or activate another protease that catalyzes the initial endoproteolytic step, as in the proteasome-dependent activation of Esp1 protease during sister chromatid exchange ( 9).	transcription
56938	3	335316	7	NULL	NULL	0	NULL	p105		nascent	released from					ribosome					NULL		NULL	NULL	NULL	NULL	gw70_science_299_5605_408_s_8	12481023	Because p50 constitutes the NH2-terminus of p105 and the COOH-terminus is presumably blocked by the ribosome, the proteasome must either wait for release of nascent p105 from the ribosome or activate another protease that catalyzes the initial endoproteolytic step, as in the proteasome-dependent activation of Esp1 protease during sister chromatid exchange ( 9).	transcription
56939	4	335316	7	NULL	NULL	0	NULL	protease			catalyze					endoproteolytic step		initial 			NULL		NULL	NULL	NULL	NULL	gw70_science_299_5605_408_s_8	12481023	Because p50 constitutes the NH2-terminus of p105 and the COOH-terminus is presumably blocked by the ribosome, the proteasome must either wait for release of nascent p105 from the ribosome or activate another protease that catalyzes the initial endoproteolytic step, as in the proteasome-dependent activation of Esp1 protease during sister chromatid exchange ( 9).	transcription
56940	5	335316	7	NULL	NULL	0	NULL	proteasome			activate					statement 4					NULL		0	NULL	NULL	NULL	gw70_science_299_5605_408_s_8	12481023	Because p50 constitutes the NH2-terminus of p105 and the COOH-terminus is presumably blocked by the ribosome, the proteasome must either wait for release of nascent p105 from the ribosome or activate another protease that catalyzes the initial endoproteolytic step, as in the proteasome-dependent activation of Esp1 protease during sister chromatid exchange ( 9).	transcription
56941	9	335316	7	NULL	NULL	0	NULL	statement 5			is an alternative to					statement 6					NULL		NULL	NULL	NULL	NULL	gw70_science_299_5605_408_s_8	12481023	Because p50 constitutes the NH2-terminus of p105 and the COOH-terminus is presumably blocked by the ribosome, the proteasome must either wait for release of nascent p105 from the ribosome or activate another protease that catalyzes the initial endoproteolytic step, as in the proteasome-dependent activation of Esp1 protease during sister chromatid exchange ( 9).	transcription
56942	7	335316	7	NULL	NULL	0	NULL	Esp1 protease		activation of	depends on					proteasome					NULL		0	NULL	NULL	NULL	gw70_science_299_5605_408_s_8	12481023	Because p50 constitutes the NH2-terminus of p105 and the COOH-terminus is presumably blocked by the ribosome, the proteasome must either wait for release of nascent p105 from the ribosome or activate another protease that catalyzes the initial endoproteolytic step, as in the proteasome-dependent activation of Esp1 protease during sister chromatid exchange ( 9).	transcription
56943	8	335316	7	NULL	NULL	0	NULL	statement 7			during					sister chromatid		exchange of			NULL		0	NULL	NULL	NULL	gw70_science_299_5605_408_s_8	12481023	Because p50 constitutes the NH2-terminus of p105 and the COOH-terminus is presumably blocked by the ribosome, the proteasome must either wait for release of nascent p105 from the ribosome or activate another protease that catalyzes the initial endoproteolytic step, as in the proteasome-dependent activation of Esp1 protease during sister chromatid exchange ( 9).	transcription
56944	6	335316	7	NULL	NULL	0	NULL	proteasome			wait for					statement 3					NULL		NULL	NULL	NULL	NULL	gw70_science_299_5605_408_s_8	12481023	Because p50 constitutes the NH2-terminus of p105 and the COOH-terminus is presumably blocked by the ribosome, the proteasome must either wait for release of nascent p105 from the ribosome or activate another protease that catalyzes the initial endoproteolytic step, as in the proteasome-dependent activation of Esp1 protease during sister chromatid exchange ( 9).	transcription
54944	1	335318	5	NULL	NULL	0	NULL				is synthesized as			p50 subunits		p105					NULL		NULL	NULL	NULL	NULL	gw70_embo_25_20_4820_s_14	16990795	The p50 and p52 subunits are synthesized as longer precursor proteins, p105 and  p100 that contain ankyrin repeats in their C-termini, similar to those possessed  by the inhibitor of NF-kappaB (IkappaB) family of proteins ( ).	transcription
54945	2	335318	5	NULL	NULL	0	NULL	p105			is a type of					long precursor protein					NULL		0	NULL	NULL	NULL	gw70_embo_25_20_4820_s_14	16990795	The p50 and p52 subunits are synthesized as longer precursor proteins, p105 and  p100 that contain ankyrin repeats in their C-termini, similar to those possessed  by the inhibitor of NF-kappaB (IkappaB) family of proteins ( ).	transcription
54946	3	335318	5	NULL	NULL	0	NULL	p105			contains					p105			ankyrin repeats in C-termini		NULL		0	NULL	NULL	NULL	gw70_embo_25_20_4820_s_14	16990795	The p50 and p52 subunits are synthesized as longer precursor proteins, p105 and  p100 that contain ankyrin repeats in their C-termini, similar to those possessed  by the inhibitor of NF-kappaB (IkappaB) family of proteins ( ).	transcription
54947	4	335318	5	NULL	NULL	0	NULL				is synthesized as			p52 subunits		p100					NULL		0	NULL	NULL	NULL	gw70_embo_25_20_4820_s_14	16990795	The p50 and p52 subunits are synthesized as longer precursor proteins, p105 and  p100 that contain ankyrin repeats in their C-termini, similar to those possessed  by the inhibitor of NF-kappaB (IkappaB) family of proteins ( ).	transcription
54948	5	335318	5	NULL	NULL	0	NULL	p100			is a type of					long precursor protein					NULL		0	NULL	NULL	NULL	gw70_embo_25_20_4820_s_14	16990795	The p50 and p52 subunits are synthesized as longer precursor proteins, p105 and  p100 that contain ankyrin repeats in their C-termini, similar to those possessed  by the inhibitor of NF-kappaB (IkappaB) family of proteins ( ).	transcription
54949	6	335318	5	NULL	NULL	0	NULL	p100			contains								ankyrin repeats in C-termini		NULL		0	NULL	NULL	NULL	gw70_embo_25_20_4820_s_14	16990795	The p50 and p52 subunits are synthesized as longer precursor proteins, p105 and  p100 that contain ankyrin repeats in their C-termini, similar to those possessed  by the inhibitor of NF-kappaB (IkappaB) family of proteins ( ).	transcription
56945	1	335318	7	NULL	NULL	0	NULL				is synthesized as			p50 subunit		p105					NULL		0	NULL	NULL	NULL	gw70_embo_25_20_4820_s_14	16990795	The p50 and p52 subunits are synthesized as longer precursor proteins, p105 and  p100 that contain ankyrin repeats in their C-termini, similar to those possessed  by the inhibitor of NF-kappaB (IkappaB) family of proteins ( ).	transcription
56946	2	335318	7	NULL	NULL	0	NULL				is synthesized as			p52 subunit		p100					NULL		0	NULL	NULL	NULL	gw70_embo_25_20_4820_s_14	16990795	The p50 and p52 subunits are synthesized as longer precursor proteins, p105 and  p100 that contain ankyrin repeats in their C-termini, similar to those possessed  by the inhibitor of NF-kappaB (IkappaB) family of proteins ( ).	transcription
56947	3	335318	7	NULL	NULL	0	NULL	p105			contains								ankyrin repeats in their C-termini		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_20_4820_s_14	16990795	The p50 and p52 subunits are synthesized as longer precursor proteins, p105 and  p100 that contain ankyrin repeats in their C-termini, similar to those possessed  by the inhibitor of NF-kappaB (IkappaB) family of proteins ( ).	transcription
56948	4	335318	7	NULL	NULL	0	NULL	p100			contains								ankyrin repeats in their C-termini		NULL		NULL	NULL	NULL	NULL	gw70_embo_25_20_4820_s_14	16990795	The p50 and p52 subunits are synthesized as longer precursor proteins, p105 and  p100 that contain ankyrin repeats in their C-termini, similar to those possessed  by the inhibitor of NF-kappaB (IkappaB) family of proteins ( ).	transcription
56949	5	335318	7	NULL	NULL	0	NULL	NF-kappaB  family		inhibitor of	contains								ankyrin repeats in their C-termini		NULL		0	NULL	NULL	NULL	gw70_embo_25_20_4820_s_14	16990795	The p50 and p52 subunits are synthesized as longer precursor proteins, p105 and  p100 that contain ankyrin repeats in their C-termini, similar to those possessed  by the inhibitor of NF-kappaB (IkappaB) family of proteins ( ).	transcription
56950	6	335318	7	NULL	NULL	0	NULL	NF-kappaB			is					IkappaB					NULL		0	NULL	NULL	NULL	gw70_embo_25_20_4820_s_14	16990795	The p50 and p52 subunits are synthesized as longer precursor proteins, p105 and  p100 that contain ankyrin repeats in their C-termini, similar to those possessed  by the inhibitor of NF-kappaB (IkappaB) family of proteins ( ).	transcription
56956	7	335318	7	NULL	NULL	0	NULL	p105			is a type of					longer precursor protein					NULL		0	NULL	NULL	NULL	gw70_embo_25_20_4820_s_14	16990795	The p50 and p52 subunits are synthesized as longer precursor proteins, p105 and  p100 that contain ankyrin repeats in their C-termini, similar to those possessed  by the inhibitor of NF-kappaB (IkappaB) family of proteins ( ).	transcription
56957	8	335318	7	NULL	NULL	0	NULL	p100			is a type of					longer precursor protein					NULL		0	NULL	NULL	NULL	gw70_embo_25_20_4820_s_14	16990795	The p50 and p52 subunits are synthesized as longer precursor proteins, p105 and  p100 that contain ankyrin repeats in their C-termini, similar to those possessed  by the inhibitor of NF-kappaB (IkappaB) family of proteins ( ).	transcription
54950	1	335319	5	NULL	NULL	0	NULL	Casper			induces					NF- B		activation of			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_4_980_s_140	13679070	Based on these data, an additional  explanation for p105-mediated inhibition of Casper-induced NF- B activation is that  Casper causes inhibition of p105 processing and subsequent lack of p50 and therefore  inhibition of NF- B activation.	transcription
54951	2	335319	5	NULL	NULL	0	NULL	p105			mediates					statement 1		inhibition of			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_4_980_s_140	13679070	Based on these data, an additional  explanation for p105-mediated inhibition of Casper-induced NF- B activation is that  Casper causes inhibition of p105 processing and subsequent lack of p50 and therefore  inhibition of NF- B activation.	transcription
54952	3	335319	5	NULL	NULL	0	NULL	Casper			inhibits					p105		processing of			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_4_980_s_140	13679070	Based on these data, an additional  explanation for p105-mediated inhibition of Casper-induced NF- B activation is that  Casper causes inhibition of p105 processing and subsequent lack of p50 and therefore  inhibition of NF- B activation.	transcription
54953	4	335319	5	NULL	NULL	0	NULL	statement 3			leads to		subsequently			p50		lack of			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_4_980_s_140	13679070	Based on these data, an additional  explanation for p105-mediated inhibition of Casper-induced NF- B activation is that  Casper causes inhibition of p105 processing and subsequent lack of p50 and therefore  inhibition of NF- B activation.	transcription
54954	5	335319	5	NULL	NULL	0	NULL	statement 4			inhibits					NF- B		activation of			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_4_980_s_140	13679070	Based on these data, an additional  explanation for p105-mediated inhibition of Casper-induced NF- B activation is that  Casper causes inhibition of p105 processing and subsequent lack of p50 and therefore  inhibition of NF- B activation.	transcription
56951	1	335319	7	NULL	NULL	0	NULL	Casper			induce					NF-B		activation of			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_4_980_s_140	13679070	Based on these data, an additional  explanation for p105-mediated inhibition of Casper-induced NF- B activation is that  Casper causes inhibition of p105 processing and subsequent lack of p50 and therefore  inhibition of NF- B activation.	transcription
56952	2	335319	7	NULL	NULL	0	NULL	Casper			inhibits					p105		processing of			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_4_980_s_140	13679070	Based on these data, an additional  explanation for p105-mediated inhibition of Casper-induced NF- B activation is that  Casper causes inhibition of p105 processing and subsequent lack of p50 and therefore  inhibition of NF- B activation.	transcription
56953	3	335319	7	NULL	NULL	0	NULL	statement 2			leads to		subsequently			p50		lack of			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_4_980_s_140	13679070	Based on these data, an additional  explanation for p105-mediated inhibition of Casper-induced NF- B activation is that  Casper causes inhibition of p105 processing and subsequent lack of p50 and therefore  inhibition of NF- B activation.	transcription
56954	4	335319	7	NULL	NULL	0	NULL	statement 3			leads to					NF-B		inhibition of;;activation of			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_4_980_s_140	13679070	Based on these data, an additional  explanation for p105-mediated inhibition of Casper-induced NF- B activation is that  Casper causes inhibition of p105 processing and subsequent lack of p50 and therefore  inhibition of NF- B activation.	transcription
56955	5	335319	7	NULL	NULL	0	NULL	p105			mediates					statement 1		inhibition of			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_309_4_980_s_140	13679070	Based on these data, an additional  explanation for p105-mediated inhibition of Casper-induced NF- B activation is that  Casper causes inhibition of p105 processing and subsequent lack of p50 and therefore  inhibition of NF- B activation.	transcription
54955	1	335320	5	NULL	NULL	0	NULL	TNF-alpha			is overexpressed by					nfkappab1 - / - HSCs					NULL		0	NULL	NULL	NULL	gw70_amjpathol_166_3_695_s_323	15743782	Overexpression of TNF-alpha by  nfkappab1 - / -  HSCs is therefore because of absence of p50 (rather than a function attributed to the precursor protein p105) and specifically arises as a consequence of the loss of p50-dependent HDAC-mediated transcriptional repression of the TNF-alpha gene.	transcription
54956	2	335320	5	NULL	NULL	0	NULL	p50		absence of	leads to					statement 1					NULL		0	NULL	NULL	NULL	gw70_amjpathol_166_3_695_s_323	15743782	Overexpression of TNF-alpha by  nfkappab1 - / -  HSCs is therefore because of absence of p50 (rather than a function attributed to the precursor protein p105) and specifically arises as a consequence of the loss of p50-dependent HDAC-mediated transcriptional repression of the TNF-alpha gene.	transcription
54957	3	335320	5	NULL	NULL	0	NULL	TNF-alpha gene		transcriptional repression of	is mediated by					HDAC					NULL		0	NULL	NULL	NULL	gw70_amjpathol_166_3_695_s_323	15743782	Overexpression of TNF-alpha by  nfkappab1 - / -  HSCs is therefore because of absence of p50 (rather than a function attributed to the precursor protein p105) and specifically arises as a consequence of the loss of p50-dependent HDAC-mediated transcriptional repression of the TNF-alpha gene.	transcription
54958	4	335320	5	NULL	NULL	0	NULL	statement 3			is dependent on					p50					NULL		0	NULL	NULL	NULL	gw70_amjpathol_166_3_695_s_323	15743782	Overexpression of TNF-alpha by  nfkappab1 - / -  HSCs is therefore because of absence of p50 (rather than a function attributed to the precursor protein p105) and specifically arises as a consequence of the loss of p50-dependent HDAC-mediated transcriptional repression of the TNF-alpha gene.	transcription
54959	5	335320	5	NULL	NULL	0	NULL	p50		loss of	leads to					statement 3		loss of			NULL		0	NULL	NULL	NULL	gw70_amjpathol_166_3_695_s_323	15743782	Overexpression of TNF-alpha by  nfkappab1 - / -  HSCs is therefore because of absence of p50 (rather than a function attributed to the precursor protein p105) and specifically arises as a consequence of the loss of p50-dependent HDAC-mediated transcriptional repression of the TNF-alpha gene.	transcription
54960	6	335320	5	NULL	NULL	0	NULL	statement 5			leads to					statement 1					NULL		0	NULL	NULL	NULL	gw70_amjpathol_166_3_695_s_323	15743782	Overexpression of TNF-alpha by  nfkappab1 - / -  HSCs is therefore because of absence of p50 (rather than a function attributed to the precursor protein p105) and specifically arises as a consequence of the loss of p50-dependent HDAC-mediated transcriptional repression of the TNF-alpha gene.	transcription
56958	1	335320	7	NULL	NULL	0	NULL	HDAC			mediate					TNF-alpha gene		transcriptional repression of 			NULL		0	NULL	NULL	NULL	gw70_amjpathol_166_3_695_s_323	15743782	Overexpression of TNF-alpha by  nfkappab1 - / -  HSCs is therefore because of absence of p50 (rather than a function attributed to the precursor protein p105) and specifically arises as a consequence of the loss of p50-dependent HDAC-mediated transcriptional repression of the TNF-alpha gene.	transcription
56959	2	335320	7	NULL	NULL	0	NULL	statement 1			depends on					p50					NULL		0	NULL	NULL	NULL	gw70_amjpathol_166_3_695_s_323	15743782	Overexpression of TNF-alpha by  nfkappab1 - / -  HSCs is therefore because of absence of p50 (rather than a function attributed to the precursor protein p105) and specifically arises as a consequence of the loss of p50-dependent HDAC-mediated transcriptional repression of the TNF-alpha gene.	transcription
56960	3	335320	7	NULL	NULL	0	NULL	nfkappab1 - / - HSCs			overexpress					TNF-alpha					NULL		0	NULL	NULL	NULL	gw70_amjpathol_166_3_695_s_323	15743782	Overexpression of TNF-alpha by  nfkappab1 - / -  HSCs is therefore because of absence of p50 (rather than a function attributed to the precursor protein p105) and specifically arises as a consequence of the loss of p50-dependent HDAC-mediated transcriptional repression of the TNF-alpha gene.	transcription
56961	4	335320	7	NULL	NULL	0	NULL	statement 3			because					p50		absence of			NULL		NULL	NULL	NULL	NULL	gw70_amjpathol_166_3_695_s_323	15743782	Overexpression of TNF-alpha by  nfkappab1 - / -  HSCs is therefore because of absence of p50 (rather than a function attributed to the precursor protein p105) and specifically arises as a consequence of the loss of p50-dependent HDAC-mediated transcriptional repression of the TNF-alpha gene.	transcription
56962	5	335320	7	NULL	NULL	0	NULL	statement 3			arises		specifically			statement 2		due to loss of			NULL		0	NULL	NULL	NULL	gw70_amjpathol_166_3_695_s_323	15743782	Overexpression of TNF-alpha by  nfkappab1 - / -  HSCs is therefore because of absence of p50 (rather than a function attributed to the precursor protein p105) and specifically arises as a consequence of the loss of p50-dependent HDAC-mediated transcriptional repression of the TNF-alpha gene.	transcription
54961	1	335321	5	NULL	NULL	0	NULL	IKK			mediates					NF- B component		phosphorylation of			NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_18_0_621_s_657	10837071	The basis for this difference in DNA-binding activity is not yet known,  although it may result from IKK -mediated phosphorylation of an NF- B component or  from an effect on the processing of p105 to p50.	transcription
54962	2	335321	5	NULL	NULL	0	NULL	p105			is processed to					p50					NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_18_0_621_s_657	10837071	The basis for this difference in DNA-binding activity is not yet known,  although it may result from IKK -mediated phosphorylation of an NF- B component or  from an effect on the processing of p105 to p50.	transcription
56963	1	335321	7	NULL	NULL	0	NULL	IKK			mediate					NF- B component		phosphorylation of			NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_18_0_621_s_657	10837071	The basis for this difference in DNA-binding activity is not yet known,  although it may result from IKK -mediated phosphorylation of an NF- B component or  from an effect on the processing of p105 to p50.	transcription
56964	2	335321	7	NULL	NULL	0	NULL	p105			processed to					p50					NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_18_0_621_s_657	10837071	The basis for this difference in DNA-binding activity is not yet known,  although it may result from IKK -mediated phosphorylation of an NF- B component or  from an effect on the processing of p105 to p50.	transcription
54963	1	335322	5	NULL	NULL	0	NULL	p105		degradation of	is mediated by					IKK					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_1_475_s_181	14673179	As was noted earlier ( ), IKK-mediated degradation of p105 results in disappearance of the cytosolic anchor of free p50 that now migrates to the nucleus (Fig.  4A, compare lane 5 to lane 3 and lane 9 to lane 7).	transcription
54964	2	335322	5	NULL	NULL	0	NULL	statement 1			results in					p50		disappearance of;;cytosolic anchor of;;free 			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_1_475_s_181	14673179	As was noted earlier ( ), IKK-mediated degradation of p105 results in disappearance of the cytosolic anchor of free p50 that now migrates to the nucleus (Fig.  4A, compare lane 5 to lane 3 and lane 9 to lane 7).	transcription
54965	3	335322	5	NULL	NULL	0	NULL	p50		free	migrates to					nucleus					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_1_475_s_181	14673179	As was noted earlier ( ), IKK-mediated degradation of p105 results in disappearance of the cytosolic anchor of free p50 that now migrates to the nucleus (Fig.  4A, compare lane 5 to lane 3 and lane 9 to lane 7).	transcription
54966	4	335322	5	NULL	NULL	0	NULL	statement 2			leads to					statement 3					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_1_475_s_181	14673179	As was noted earlier ( ), IKK-mediated degradation of p105 results in disappearance of the cytosolic anchor of free p50 that now migrates to the nucleus (Fig.  4A, compare lane 5 to lane 3 and lane 9 to lane 7).	transcription
56965	1	335322	7	NULL	NULL	0	NULL	IKK			mediates					p105		degradation of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_1_475_s_181	14673179	As was noted earlier ( ), IKK-mediated degradation of p105 results in disappearance of the cytosolic anchor of free p50 that now migrates to the nucleus (Fig.  4A, compare lane 5 to lane 3 and lane 9 to lane 7).	transcription
56966	2	335322	7	NULL	NULL	0	NULL	statement 1			result in					free p50		disappearance of 	 cytosolic anchor of		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_1_475_s_181	14673179	As was noted earlier ( ), IKK-mediated degradation of p105 results in disappearance of the cytosolic anchor of free p50 that now migrates to the nucleus (Fig.  4A, compare lane 5 to lane 3 and lane 9 to lane 7).	transcription
56967	3	335322	7	NULL	NULL	0	NULL	p50			migrates to					nucleus					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_1_475_s_181	14673179	As was noted earlier ( ), IKK-mediated degradation of p105 results in disappearance of the cytosolic anchor of free p50 that now migrates to the nucleus (Fig.  4A, compare lane 5 to lane 3 and lane 9 to lane 7).	transcription
56968	4	335322	7	NULL	NULL	0	NULL	statement 2			leads to					statement 3					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_1_475_s_181	14673179	As was noted earlier ( ), IKK-mediated degradation of p105 results in disappearance of the cytosolic anchor of free p50 that now migrates to the nucleus (Fig.  4A, compare lane 5 to lane 3 and lane 9 to lane 7).	transcription
56969	1	335323	7	NULL	NULL	0	NULL	Kinase			process		rapidly			p105		synthesized			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_1_475_s_203	14673179	The reason is that during the 24 h of transfection in the presence of IKKbeta that precedes the analysis, the synthesized p105 is rapidly processed and degraded under the effect of the kinase, and a stable p50 is accumulated continuously.	transcription
56970	2	335323	7	NULL	NULL	0	NULL	kinase			degrades		rapidly			statement 1					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_1_475_s_203	14673179	The reason is that during the 24 h of transfection in the presence of IKKbeta that precedes the analysis, the synthesized p105 is rapidly processed and degraded under the effect of the kinase, and a stable p50 is accumulated continuously.	transcription
56971	3	335323	7	NULL	NULL	0	NULL	statement 2			leads to					p50		continuous accumulation of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_1_475_s_203	14673179	The reason is that during the 24 h of transfection in the presence of IKKbeta that precedes the analysis, the synthesized p105 is rapidly processed and degraded under the effect of the kinase, and a stable p50 is accumulated continuously.	transcription
56097	1	335324	6	NULL	NULL	0	NULL	IKKbeta		stimulation by	results in					p105		complete degradation of 			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_1_475_s_310	14673179	Heissmeyer and colleagues ( ,  ) have shown that stimulation by IKKbeta with subsequent ubiquitination by beta-TrCP results in almost complete degradation of p105, while the increased generation of p50 is slight and inconsistent.	transcription
56098	2	335324	6	NULL	NULL	0	NULL	beta-TrCP		ubiquitination by	results in					p105		complete degradation of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_1_475_s_310	14673179	Heissmeyer and colleagues ( ,  ) have shown that stimulation by IKKbeta with subsequent ubiquitination by beta-TrCP results in almost complete degradation of p105, while the increased generation of p50 is slight and inconsistent.	transcription
56972	1	335324	7	NULL	NULL	0	NULL	IKKbeta		stimulation by	results in					p105		complete degradation of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_1_475_s_310	14673179	Heissmeyer and colleagues ( ,  ) have shown that stimulation by IKKbeta with subsequent ubiquitination by beta-TrCP results in almost complete degradation of p105, while the increased generation of p50 is slight and inconsistent.	transcription
56973	2	335324	7	NULL	NULL	0	NULL	beta-TrCP		ubiquitination by	results in					p105		complete degradation of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_1_475_s_310	14673179	Heissmeyer and colleagues ( ,  ) have shown that stimulation by IKKbeta with subsequent ubiquitination by beta-TrCP results in almost complete degradation of p105, while the increased generation of p50 is slight and inconsistent.	transcription
56974	3	335324	7	NULL	NULL	0	NULL	statement 1			occur simulataneous with					statement 2					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_1_475_s_310	14673179	Heissmeyer and colleagues ( ,  ) have shown that stimulation by IKKbeta with subsequent ubiquitination by beta-TrCP results in almost complete degradation of p105, while the increased generation of p50 is slight and inconsistent.	transcription
56975	4	335324	7	NULL	NULL	0	NULL	statement 3			leads to					p50		slightly increased generation of 			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_1_475_s_310	14673179	Heissmeyer and colleagues ( ,  ) have shown that stimulation by IKKbeta with subsequent ubiquitination by beta-TrCP results in almost complete degradation of p105, while the increased generation of p50 is slight and inconsistent.	transcription
56976	5	335324	7	NULL	NULL	0	NULL	statement 3			leads to					p50		inconsistent generation of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_1_475_s_310	14673179	Heissmeyer and colleagues ( ,  ) have shown that stimulation by IKKbeta with subsequent ubiquitination by beta-TrCP results in almost complete degradation of p105, while the increased generation of p50 is slight and inconsistent.	transcription
56977	1	335325	7	NULL	NULL	0	NULL	 p105 heterodimers			recruits		non-proteolytically			p50					NULL	cytosol	0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8460_s_290	14668329	The induction of Bcl-3 in tolerant T cells may be relevant in the nuclear shuttling of p50-p50 homodimers, which could be the result from a non-proteolytic recruitment of p50 from p105 heterodimers in the cytosol.	transcription
56978	2	335325	7	NULL	NULL	0	NULL	Bcl-3		 induction of 	relevant in		may be			p50-p50 homodimers		nuclear shuttling of			NULL	tolerant T cells	0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8460_s_290	14668329	The induction of Bcl-3 in tolerant T cells may be relevant in the nuclear shuttling of p50-p50 homodimers, which could be the result from a non-proteolytic recruitment of p50 from p105 heterodimers in the cytosol.	transcription
56979	3	335325	7	NULL	NULL	0	NULL	statement 2			result from					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8460_s_290	14668329	The induction of Bcl-3 in tolerant T cells may be relevant in the nuclear shuttling of p50-p50 homodimers, which could be the result from a non-proteolytic recruitment of p50 from p105 heterodimers in the cytosol.	transcription
56099	1	335326	6	NULL	NULL	0	NULL	MEK/ERK pathway		activation of	controls					p105		processing of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_32465_s_189	12801933	By a similar mechanism,  the constitutive p50 homodimer signal in LY-ar cells may not be a result of  MEK/ERK-induced Bcl-3 activity but rather a result of increased p105  processing directly or indirectly controlled by activation of the MEK/ERK  pathway.	transcription
56980	1	335326	7	NULL	NULL	0	NULL	MEK/ERK			induce					Bcl-3		activity of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_32465_s_189	12801933	By a similar mechanism,  the constitutive p50 homodimer signal in LY-ar cells may not be a result of  MEK/ERK-induced Bcl-3 activity but rather a result of increased p105  processing directly or indirectly controlled by activation of the MEK/ERK  pathway.	transcription
56981	2	335326	7	NULL	NULL	0	NULL	statement 1			does not result in					p50 homodimer		constitutive signal of			NULL	LY-ar cells	0	NULL	NULL	NULL	gw70_jbiolchem_278_34_32465_s_189	12801933	By a similar mechanism,  the constitutive p50 homodimer signal in LY-ar cells may not be a result of  MEK/ERK-induced Bcl-3 activity but rather a result of increased p105  processing directly or indirectly controlled by activation of the MEK/ERK  pathway.	transcription
56982	3	335326	7	NULL	NULL	0	NULL	MEK/ERK pathway		activation of	controls		directly			p105		increased processing of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_32465_s_189	12801933	By a similar mechanism,  the constitutive p50 homodimer signal in LY-ar cells may not be a result of  MEK/ERK-induced Bcl-3 activity but rather a result of increased p105  processing directly or indirectly controlled by activation of the MEK/ERK  pathway.	transcription
56983	4	335326	7	NULL	NULL	0	NULL	MEK/ERK pathway		activation of	controls		indirectly			p105		increased processing of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_32465_s_189	12801933	By a similar mechanism,  the constitutive p50 homodimer signal in LY-ar cells may not be a result of  MEK/ERK-induced Bcl-3 activity but rather a result of increased p105  processing directly or indirectly controlled by activation of the MEK/ERK  pathway.	transcription
56984	5	335326	7	NULL	NULL	0	NULL	statement 3			is an alternative to					statement 4					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_32465_s_189	12801933	By a similar mechanism,  the constitutive p50 homodimer signal in LY-ar cells may not be a result of  MEK/ERK-induced Bcl-3 activity but rather a result of increased p105  processing directly or indirectly controlled by activation of the MEK/ERK  pathway.	transcription
56985	6	335326	7	NULL	NULL	0	NULL	statement 5			result in					p50 homodimer		constitutive signal of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_34_32465_s_189	12801933	By a similar mechanism,  the constitutive p50 homodimer signal in LY-ar cells may not be a result of  MEK/ERK-induced Bcl-3 activity but rather a result of increased p105  processing directly or indirectly controlled by activation of the MEK/ERK  pathway.	transcription
56100	1	335327	6	NULL	NULL	0	NULL	NF-kappaB			is sequestered to					cytoplasm					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
56101	2	335327	6	NULL	NULL	0	NULL	IkappaB			performs					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
56102	3	335327	6	NULL	NULL	0	NULL	p105			performs					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
56103	4	335327	6	NULL	NULL	0	NULL	p100			performs					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
56104	5	335327	6	NULL	NULL	0	NULL	p105			is a type of					NF-kappaB precursor protein					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
56105	6	335327	6	NULL	NULL	0	NULL	p100			is a type of					NF-kappaB precursor protein					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
56986	1	335327	7	NULL	NULL	0	NULL	NF-kappaB 			is composed of					p50 dimer					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
56987	2	335327	7	NULL	NULL	0	NULL	NF-kappaB 			is composed of					p52 dimer					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
56988	3	335327	7	NULL	NULL	0	NULL	NF-kappaB 			is composed of					RelA dimer					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
56989	4	335327	7	NULL	NULL	0	NULL	NF-kappaB			is composed of					RelB dimer					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
56990	5	335327	7	NULL	NULL	0	NULL	NF-kappaB			is composed of					c-Rel dimer					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
56991	6	335327	7	NULL	NULL	0	NULL	p50 dimer			complexed to		endogenously			p105					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
56992	7	335327	7	NULL	NULL	0	NULL	p50 dimer			complexed to		endogenously			p100					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
56993	8	335327	7	NULL	NULL	0	NULL	p52 dimer			complexed to		endogenously			p105					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
56994	9	335327	7	NULL	NULL	0	NULL	p52 dimer			complexed to		endogenously			p100					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
56995	10	335327	7	NULL	NULL	0	NULL	RelA dimer			complexed to		endogenously			p105					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
56996	11	335327	7	NULL	NULL	0	NULL	RelA dimer			complexed to		endogenously			p100					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
56997	12	335327	7	NULL	NULL	0	NULL	RelB dimer			complexed to		endogenously			p105					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
56998	13	335327	7	NULL	NULL	0	NULL	RelB dimer			complexed to		endogenously			p100					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
56999	14	335327	7	NULL	NULL	0	NULL	c-Rel dimer			complexed to		endogenously			p105					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
57000	15	335327	7	NULL	NULL	0	NULL	c-Rel dimer			complexed to		endogenously			p100					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
57001	16	335327	7	NULL	NULL	0	NULL	p105			is a precursor of					IkappaB protein					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
57002	17	335327	7	NULL	NULL	0	NULL	p105			is a precursor of					NF-kappaB protein					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
57003	18	335327	7	NULL	NULL	0	NULL	p100			is a precursor of					IkappaB protein					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
57004	19	335327	7	NULL	NULL	0	NULL	p100			is a precursor of					NF-kappaB protein					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
57005	20	335327	7	NULL	NULL	0	NULL	IkappaB			is a type of					inhibitory protein					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
57006	21	335327	7	NULL	NULL	0	NULL	NF-kappaB			is a type of					inhibitory protein					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
57007	22	335327	7	NULL	NULL	0	NULL	p105			sequester					NF-kappaB					NULL	cytoplasm	0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
57008	23	335327	7	NULL	NULL	0	NULL	p100			sequester					NF-kappaB					NULL	cytoplasm	0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
57017	24	335327	7	NULL	NULL	0	NULL	statement 6			is an alternative to					statement 7					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
57018	25	335327	7	NULL	NULL	0	NULL	statement 8			is an alternative to					statement 9					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
57019	26	335327	7	NULL	NULL	0	NULL	statement 10			is an alternative to					statement 11					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
57020	27	335327	7	NULL	NULL	0	NULL	statement 12			is an alternative to					statement 13					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
57021	28	335327	7	NULL	NULL	0	NULL	statement 14			is an alternative to					statement 15					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_47_46565_s_17	12968033	NF-kappaB is composed of dimers of p50, p52, RelA, RelB, or c-Rel that are endogenously complexed to inhibitor proteins called IkappaB and NF-kappaB precursor proteins p105 or p100, which sequester NF-kappaB in the cytoplasm.	transcription
56106	1	335328	6	NULL	NULL	0	NULL	p50			interacts with					IkappaBalpha					NULL		0	NULL	NULL	NULL	gw70_pnas_103_40_14767_s_135	17003112	Manipulations of FIH levels in this setting resulted in no major effects on interactions of p50 with either IkappaBalpha or p105, on nuclear abundance of the proteins, or on NF-kappaB DNA-binding activity (data not shown).	transcription
56107	2	335328	6	NULL	NULL	0	NULL	p50			interacts with					p105					NULL		0	NULL	NULL	NULL	gw70_pnas_103_40_14767_s_135	17003112	Manipulations of FIH levels in this setting resulted in no major effects on interactions of p50 with either IkappaBalpha or p105, on nuclear abundance of the proteins, or on NF-kappaB DNA-binding activity (data not shown).	transcription
56108	3	335328	6	NULL	NULL	0	NULL	statement 1			is an alternative to					statement 2					NULL		0	NULL	NULL	NULL	gw70_pnas_103_40_14767_s_135	17003112	Manipulations of FIH levels in this setting resulted in no major effects on interactions of p50 with either IkappaBalpha or p105, on nuclear abundance of the proteins, or on NF-kappaB DNA-binding activity (data not shown).	transcription
57009	1	335328	7	NULL	NULL	0	NULL	p50			interacts with					IkappaBalpha					NULL		0	NULL	NULL	NULL	gw70_pnas_103_40_14767_s_135	17003112	Manipulations of FIH levels in this setting resulted in no major effects on interactions of p50 with either IkappaBalpha or p105, on nuclear abundance of the proteins, or on NF-kappaB DNA-binding activity (data not shown).	transcription
57010	2	335328	7	NULL	NULL	0	NULL	p50			interacts with					p105					NULL		0	NULL	NULL	NULL	gw70_pnas_103_40_14767_s_135	17003112	Manipulations of FIH levels in this setting resulted in no major effects on interactions of p50 with either IkappaBalpha or p105, on nuclear abundance of the proteins, or on NF-kappaB DNA-binding activity (data not shown).	transcription
57011	3	335328	7	NULL	NULL	0	NULL	FIH		levels of	does not effect					statement 1					NULL		0	NULL	NULL	NULL	gw70_pnas_103_40_14767_s_135	17003112	Manipulations of FIH levels in this setting resulted in no major effects on interactions of p50 with either IkappaBalpha or p105, on nuclear abundance of the proteins, or on NF-kappaB DNA-binding activity (data not shown).	transcription
57012	4	335328	7	NULL	NULL	0	NULL	FIH		levels of	does not effect					statement 2					NULL		0	NULL	NULL	NULL	gw70_pnas_103_40_14767_s_135	17003112	Manipulations of FIH levels in this setting resulted in no major effects on interactions of p50 with either IkappaBalpha or p105, on nuclear abundance of the proteins, or on NF-kappaB DNA-binding activity (data not shown).	transcription
57013	5	335328	7	NULL	NULL	0	NULL	FIH		levels of	does not effect on					proteins		nuclear abundance of			NULL		0	NULL	NULL	NULL	gw70_pnas_103_40_14767_s_135	17003112	Manipulations of FIH levels in this setting resulted in no major effects on interactions of p50 with either IkappaBalpha or p105, on nuclear abundance of the proteins, or on NF-kappaB DNA-binding activity (data not shown).	transcription
57014	6	335328	7	NULL	NULL	0	NULL	NF-kappaB			bind					DNA					NULL		0	NULL	NULL	NULL	gw70_pnas_103_40_14767_s_135	17003112	Manipulations of FIH levels in this setting resulted in no major effects on interactions of p50 with either IkappaBalpha or p105, on nuclear abundance of the proteins, or on NF-kappaB DNA-binding activity (data not shown).	transcription
57015	7	335328	7	NULL	NULL	0	NULL	FIH		levels of	does not effect					statement 6					NULL		0	NULL	NULL	NULL	gw70_pnas_103_40_14767_s_135	17003112	Manipulations of FIH levels in this setting resulted in no major effects on interactions of p50 with either IkappaBalpha or p105, on nuclear abundance of the proteins, or on NF-kappaB DNA-binding activity (data not shown).	transcription
57016	8	335328	7	NULL	NULL	0	NULL	statement 3			is an alternative to					statement 4					NULL		0	NULL	NULL	NULL	gw70_pnas_103_40_14767_s_135	17003112	Manipulations of FIH levels in this setting resulted in no major effects on interactions of p50 with either IkappaBalpha or p105, on nuclear abundance of the proteins, or on NF-kappaB DNA-binding activity (data not shown).	transcription
77626	1	335329	6	NULL	NULL	0	NULL	p100 	GP		processes into					p52	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_1_141_s_29	14691250	LMP1 induces p100 and p105 NF-kappaB precursors and up-regulates their processing into p52 and p50, respectively ( ), implicating LMP1 in both canonical NF-kappaB up-regulation and noncanonical p100 processing into p52.	transcription
77627	2	335329	6	NULL	NULL	0	NULL	p105	GP		processes into					p50	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_1_141_s_29	14691250	LMP1 induces p100 and p105 NF-kappaB precursors and up-regulates their processing into p52 and p50, respectively ( ), implicating LMP1 in both canonical NF-kappaB up-regulation and noncanonical p100 processing into p52.	transcription
77628	3	335329	6	NULL	NULL	0	NULL	p100	GP		is a type of					NF-kappaB precursor	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_1_141_s_29	14691250	LMP1 induces p100 and p105 NF-kappaB precursors and up-regulates their processing into p52 and p50, respectively ( ), implicating LMP1 in both canonical NF-kappaB up-regulation and noncanonical p100 processing into p52.	transcription
77629	4	335329	6	NULL	NULL	0	NULL	p105	GP		is a type of					NF-kappaB precursor	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_1_141_s_29	14691250	LMP1 induces p100 and p105 NF-kappaB precursors and up-regulates their processing into p52 and p50, respectively ( ), implicating LMP1 in both canonical NF-kappaB up-regulation and noncanonical p100 processing into p52.	transcription
77630	5	335329	6	NULL	NULL	0	NULL	LMP1	GP		induces					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_101_1_141_s_29	14691250	LMP1 induces p100 and p105 NF-kappaB precursors and up-regulates their processing into p52 and p50, respectively ( ), implicating LMP1 in both canonical NF-kappaB up-regulation and noncanonical p100 processing into p52.	transcription
57022	1	335329	7	NULL	NULL	0	NULL	p100			processed to					p52					NULL		0	NULL	NULL	NULL	gw70_pnas_101_1_141_s_29	14691250	LMP1 induces p100 and p105 NF-kappaB precursors and up-regulates their processing into p52 and p50, respectively ( ), implicating LMP1 in both canonical NF-kappaB up-regulation and noncanonical p100 processing into p52.	transcription
57023	2	335329	7	NULL	NULL	0	NULL	p105			processed to					p50					NULL		0	NULL	NULL	NULL	gw70_pnas_101_1_141_s_29	14691250	LMP1 induces p100 and p105 NF-kappaB precursors and up-regulates their processing into p52 and p50, respectively ( ), implicating LMP1 in both canonical NF-kappaB up-regulation and noncanonical p100 processing into p52.	transcription
57024	3	335329	7	NULL	NULL	0	NULL	LMP1			induce					p100					NULL		0	NULL	NULL	NULL	gw70_pnas_101_1_141_s_29	14691250	LMP1 induces p100 and p105 NF-kappaB precursors and up-regulates their processing into p52 and p50, respectively ( ), implicating LMP1 in both canonical NF-kappaB up-regulation and noncanonical p100 processing into p52.	transcription
57025	4	335329	7	NULL	NULL	0	NULL	LMP1			induce					p105					NULL		0	NULL	NULL	NULL	gw70_pnas_101_1_141_s_29	14691250	LMP1 induces p100 and p105 NF-kappaB precursors and up-regulates their processing into p52 and p50, respectively ( ), implicating LMP1 in both canonical NF-kappaB up-regulation and noncanonical p100 processing into p52.	transcription
57026	5	335329	7	NULL	NULL	0	NULL	LMP1			upregulates					statement 1					NULL		0	NULL	NULL	NULL	gw70_pnas_101_1_141_s_29	14691250	LMP1 induces p100 and p105 NF-kappaB precursors and up-regulates their processing into p52 and p50, respectively ( ), implicating LMP1 in both canonical NF-kappaB up-regulation and noncanonical p100 processing into p52.	transcription
57027	6	335329	7	NULL	NULL	0	NULL	LMP1			upregulates					statement 2					NULL		0	NULL	NULL	NULL	gw70_pnas_101_1_141_s_29	14691250	LMP1 induces p100 and p105 NF-kappaB precursors and up-regulates their processing into p52 and p50, respectively ( ), implicating LMP1 in both canonical NF-kappaB up-regulation and noncanonical p100 processing into p52.	transcription
57028	7	335329	7	NULL	NULL	0	NULL	LMP1			implicated in					NF-kappaB		up-regulation of;;canonical			NULL		0	NULL	NULL	NULL	gw70_pnas_101_1_141_s_29	14691250	LMP1 induces p100 and p105 NF-kappaB precursors and up-regulates their processing into p52 and p50, respectively ( ), implicating LMP1 in both canonical NF-kappaB up-regulation and noncanonical p100 processing into p52.	transcription
57029	8	335329	7	NULL	NULL	0	NULL	LMP1			implicated in					statement 1		noncanonical			NULL		0	NULL	NULL	NULL	gw70_pnas_101_1_141_s_29	14691250	LMP1 induces p100 and p105 NF-kappaB precursors and up-regulates their processing into p52 and p50, respectively ( ), implicating LMP1 in both canonical NF-kappaB up-regulation and noncanonical p100 processing into p52.	transcription
57030	9	335329	7	NULL	NULL	0	NULL	p100			is a type of					NF-kappaB precursor					NULL		0	NULL	NULL	NULL	gw70_pnas_101_1_141_s_29	14691250	LMP1 induces p100 and p105 NF-kappaB precursors and up-regulates their processing into p52 and p50, respectively ( ), implicating LMP1 in both canonical NF-kappaB up-regulation and noncanonical p100 processing into p52.	transcription
57031	10	335329	7	NULL	NULL	0	NULL	p105			is a type of					NF-kappaB precursor					NULL		0	NULL	NULL	NULL	gw70_pnas_101_1_141_s_29	14691250	LMP1 induces p100 and p105 NF-kappaB precursors and up-regulates their processing into p52 and p50, respectively ( ), implicating LMP1 in both canonical NF-kappaB up-regulation and noncanonical p100 processing into p52.	transcription
77631	1	335330	6	NULL	NULL	0	NULL	p105	GP		modulates					p50 homodimer	GP				NULL	in vivo	0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_254	10970863	p105 modulates p50 homodimer in vivo   The formation of homo- or heterodimers is a common intracellular event involving many proteins; however, the rules that regulate such assemblies are not well understood ( Lamb and McKnight, 1991;  Tjian and Maniatis, 1994).	transcription
57032	1	335330	7	NULL	NULL	0	NULL	p105			modulate					p50 homodimer					NULL	in vivo	0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_254	10970863	p105 modulates p50 homodimer in vivo   The formation of homo- or heterodimers is a common intracellular event involving many proteins; however, the rules that regulate such assemblies are not well understood ( Lamb and McKnight, 1991;  Tjian and Maniatis, 1994).	transcription
57033	2	335330	7	NULL	NULL	0	NULL	homo-dimer		formation of	is a type of					intracellular event					NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_254	10970863	p105 modulates p50 homodimer in vivo   The formation of homo- or heterodimers is a common intracellular event involving many proteins; however, the rules that regulate such assemblies are not well understood ( Lamb and McKnight, 1991;  Tjian and Maniatis, 1994).	transcription
57034	3	335330	7	NULL	NULL	0	NULL	heterodimer		formation of	is a type of					intracellular event					NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_254	10970863	p105 modulates p50 homodimer in vivo   The formation of homo- or heterodimers is a common intracellular event involving many proteins; however, the rules that regulate such assemblies are not well understood ( Lamb and McKnight, 1991;  Tjian and Maniatis, 1994).	transcription
78185	1	335331	6	NULL	NULL	0	NULL	BCL-3	GP		is a type of					oncoprotein	GP				NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_483	10970863	Watanabe,N., Iwamura,T., Shinoda,T. and Fujita,T. (1997) Regulation of NF-kappaB1 proteins by candidate oncoprotein BCL-3: generation of NF-kappaB homodimers from the cytoplasmic pool of p50 - p105 and nuclear translocation.	transcription
78186	2	335331	6	NULL	NULL	0	NULL	BCL-3	GP		regulate					NF-kappaB1 proteins	GP				NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_483	10970863	Watanabe,N., Iwamura,T., Shinoda,T. and Fujita,T. (1997) Regulation of NF-kappaB1 proteins by candidate oncoprotein BCL-3: generation of NF-kappaB homodimers from the cytoplasmic pool of p50 - p105 and nuclear translocation.	transcription
57035	1	335331	7	NULL	NULL	0	NULL	BCL-3			regulate					NF-kappaB1 protein					NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_483	10970863	Watanabe,N., Iwamura,T., Shinoda,T. and Fujita,T. (1997) Regulation of NF-kappaB1 proteins by candidate oncoprotein BCL-3: generation of NF-kappaB homodimers from the cytoplasmic pool of p50 - p105 and nuclear translocation.	transcription
57036	2	335331	7	NULL	NULL	0	NULL	BCL-3			is a type of					oncoprotein					NULL		NULL	NULL	NULL	NULL	gw60_embo_19_17_4712_s_483	10970863	Watanabe,N., Iwamura,T., Shinoda,T. and Fujita,T. (1997) Regulation of NF-kappaB1 proteins by candidate oncoprotein BCL-3: generation of NF-kappaB homodimers from the cytoplasmic pool of p50 - p105 and nuclear translocation.	transcription
78187	1	335332	6	NULL	NULL	0	NULL	TNF-alpha	GP		induces					p105	GP	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_198	10469655	The finding that TNF-alpha induces p105 phosphorylation by IKKalpha (Figures  4 and  5) suggests that this is a rate-limiting step for precursor proteolysis and release of p50 or other associated NF-kappaB subunits.	transcription
78188	2	335332	6	NULL	NULL	0	NULL	statement 1	process		occurs by					IKKalpha	GP				NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_198	10469655	The finding that TNF-alpha induces p105 phosphorylation by IKKalpha (Figures  4 and  5) suggests that this is a rate-limiting step for precursor proteolysis and release of p50 or other associated NF-kappaB subunits.	transcription
57037	1	335332	7	NULL	NULL	0	NULL	IKKalpha 			phosphorylates					p105					NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_198	10469655	The finding that TNF-alpha induces p105 phosphorylation by IKKalpha (Figures  4 and  5) suggests that this is a rate-limiting step for precursor proteolysis and release of p50 or other associated NF-kappaB subunits.	transcription
57038	2	335332	7	NULL	NULL	0	NULL	TNF-alpha			induce					statement 1					NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_198	10469655	The finding that TNF-alpha induces p105 phosphorylation by IKKalpha (Figures  4 and  5) suggests that this is a rate-limiting step for precursor proteolysis and release of p50 or other associated NF-kappaB subunits.	transcription
57039	3	335332	7	NULL	NULL	0	NULL	statement 2			rate limiting step for					precursor		 proteolysis of			NULL		NULL	NULL	NULL	NULL	gw60_embo_18_17_4766_s_198	10469655	The finding that TNF-alpha induces p105 phosphorylation by IKKalpha (Figures  4 and  5) suggests that this is a rate-limiting step for precursor proteolysis and release of p50 or other associated NF-kappaB subunits.	transcription
57040	4	335332	7	NULL	NULL	0	NULL	statement 2			rate limiting step for					p50		release of			NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_198	10469655	The finding that TNF-alpha induces p105 phosphorylation by IKKalpha (Figures  4 and  5) suggests that this is a rate-limiting step for precursor proteolysis and release of p50 or other associated NF-kappaB subunits.	transcription
57041	5	335332	7	NULL	NULL	0	NULL	statement 2			rate limiting step for					NF-kappaB			subunits		NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_198	10469655	The finding that TNF-alpha induces p105 phosphorylation by IKKalpha (Figures  4 and  5) suggests that this is a rate-limiting step for precursor proteolysis and release of p50 or other associated NF-kappaB subunits.	transcription
57042	1	335333	7	NULL	NULL	0	NULL	MEFs			lack					p105			C-terminal ankyrin domain of 		NULL		0	NULL	NULL	NULL	gw60_embo_22_1_121_s_152	12505990	In striking contrast, kappaB binding in MEFs from mice lacking the C-terminal ankyrin domain of p105, but still expressing p50 ( Ishikawa  et al., 1998), consisted almost exclusively of RelA complexes (Figure  7A).	transcription
57043	2	335333	7	NULL	NULL	0	NULL	MEFs			express					p50 					NULL		0	NULL	NULL	NULL	gw60_embo_22_1_121_s_152	12505990	In striking contrast, kappaB binding in MEFs from mice lacking the C-terminal ankyrin domain of p105, but still expressing p50 ( Ishikawa  et al., 1998), consisted almost exclusively of RelA complexes (Figure  7A).	transcription
57044	3	335333	7	NULL	NULL	0	NULL	MEFs			consist					RelA complexes		exclusively of			NULL		0	NULL	NULL	NULL	gw60_embo_22_1_121_s_152	12505990	In striking contrast, kappaB binding in MEFs from mice lacking the C-terminal ankyrin domain of p105, but still expressing p50 ( Ishikawa  et al., 1998), consisted almost exclusively of RelA complexes (Figure  7A).	transcription
57045	4	335333	7	NULL	NULL	0	NULL	kappaB		binding of	occur in 					MEFs					NULL		0	NULL	NULL	NULL	gw60_embo_22_1_121_s_152	12505990	In striking contrast, kappaB binding in MEFs from mice lacking the C-terminal ankyrin domain of p105, but still expressing p50 ( Ishikawa  et al., 1998), consisted almost exclusively of RelA complexes (Figure  7A).	transcription
78189	1	335334	6	NULL	NULL	0	NULL	CER	GP		activates					AP1	GP				NULL		0	NULL	NULL	NULL	gw60_febslett_507_2_163_s_160	11684091	It has been reported that CER activates AP1 by increasing c-jun mRNA synthesis [  27], or NF- B by inducing the processing of p105 to p50, a component of the NF- B transcription factor [  28].	transcription
78190	2	335334	6	NULL	NULL	0	NULL	CER	GP		increases					c-jun mRNA	NucleicAcid	synthesis of			NULL		0	NULL	NULL	NULL	gw60_febslett_507_2_163_s_160	11684091	It has been reported that CER activates AP1 by increasing c-jun mRNA synthesis [  27], or NF- B by inducing the processing of p105 to p50, a component of the NF- B transcription factor [  28].	transcription
78191	3	335334	6	NULL	NULL	0	NULL	p105	GP		is processed to					p50	GP				NULL		0	NULL	NULL	NULL	gw60_febslett_507_2_163_s_160	11684091	It has been reported that CER activates AP1 by increasing c-jun mRNA synthesis [  27], or NF- B by inducing the processing of p105 to p50, a component of the NF- B transcription factor [  28].	transcription
78192	4	335334	6	NULL	NULL	0	NULL	CER	GP		activates					NF-B	GP				NULL		0	NULL	NULL	NULL	gw60_febslett_507_2_163_s_160	11684091	It has been reported that CER activates AP1 by increasing c-jun mRNA synthesis [  27], or NF- B by inducing the processing of p105 to p50, a component of the NF- B transcription factor [  28].	transcription
78193	5	335334	6	NULL	NULL	0	NULL	statement 4	process		occurs via					statement 3	process				NULL		0	NULL	NULL	NULL	gw60_febslett_507_2_163_s_160	11684091	It has been reported that CER activates AP1 by increasing c-jun mRNA synthesis [  27], or NF- B by inducing the processing of p105 to p50, a component of the NF- B transcription factor [  28].	transcription
57046	1	335334	7	NULL	NULL	0	NULL	CER			activates					AP1					NULL		0	NULL	NULL	NULL	gw60_febslett_507_2_163_s_160	11684091	It has been reported that CER activates AP1 by increasing c-jun mRNA synthesis [  27], or NF- B by inducing the processing of p105 to p50, a component of the NF- B transcription factor [  28].	transcription
57047	2	335334	7	NULL	NULL	0	NULL	statement 1			occur by					c-jun mRNA		increasing synthesis of			NULL		0	NULL	NULL	NULL	gw60_febslett_507_2_163_s_160	11684091	It has been reported that CER activates AP1 by increasing c-jun mRNA synthesis [  27], or NF- B by inducing the processing of p105 to p50, a component of the NF- B transcription factor [  28].	transcription
57048	3	335334	7	NULL	NULL	0	NULL	statement 1			occur through					NF-B					NULL		NULL	NULL	NULL	NULL	gw60_febslett_507_2_163_s_160	11684091	It has been reported that CER activates AP1 by increasing c-jun mRNA synthesis [  27], or NF- B by inducing the processing of p105 to p50, a component of the NF- B transcription factor [  28].	transcription
57049	4	335334	7	NULL	NULL	0	NULL	p105			processed to					p50					NULL		0	NULL	NULL	NULL	gw60_febslett_507_2_163_s_160	11684091	It has been reported that CER activates AP1 by increasing c-jun mRNA synthesis [  27], or NF- B by inducing the processing of p105 to p50, a component of the NF- B transcription factor [  28].	transcription
57050	5	335334	7	NULL	NULL	0	NULL	statement 3			occur by					statement 4		inducing			NULL		0	NULL	NULL	NULL	gw60_febslett_507_2_163_s_160	11684091	It has been reported that CER activates AP1 by increasing c-jun mRNA synthesis [  27], or NF- B by inducing the processing of p105 to p50, a component of the NF- B transcription factor [  28].	transcription
57051	6	335334	7	NULL	NULL	0	NULL	p50			is a component of					NF- B transcription factor					NULL		0	NULL	NULL	NULL	gw60_febslett_507_2_163_s_160	11684091	It has been reported that CER activates AP1 by increasing c-jun mRNA synthesis [  27], or NF- B by inducing the processing of p105 to p50, a component of the NF- B transcription factor [  28].	transcription
78194	1	335335	6	NULL	NULL	0	NULL	ASMase	GP		activate		may			I B kinase complex	OrganismPart				NULL		0	NULL	NULL	NULL	gw60_febslett_526_1_15_s_180	12208496	Hence, it is conceivable that ASMase may activate the I B kinase complex, which in turn leads to phosphorylation and proteasome-limited proteolysis of p105, the precursor form of p50 [  39].	transcription
78195	2	335335	6	NULL	NULL	0	NULL	statement 1	process		leads to					p105	GP	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_febslett_526_1_15_s_180	12208496	Hence, it is conceivable that ASMase may activate the I B kinase complex, which in turn leads to phosphorylation and proteasome-limited proteolysis of p105, the precursor form of p50 [  39].	transcription
78196	3	335335	6	NULL	NULL	0	NULL	statement 1	process		leads to					p105	GP	proteolysis of			NULL		0	NULL	NULL	NULL	gw60_febslett_526_1_15_s_180	12208496	Hence, it is conceivable that ASMase may activate the I B kinase complex, which in turn leads to phosphorylation and proteasome-limited proteolysis of p105, the precursor form of p50 [  39].	transcription
78197	4	335335	6	NULL	NULL	0	NULL	p105	GP	proteolysis of	is limited to					proteasome	CellComponent				NULL		0	NULL	NULL	NULL	gw60_febslett_526_1_15_s_180	12208496	Hence, it is conceivable that ASMase may activate the I B kinase complex, which in turn leads to phosphorylation and proteasome-limited proteolysis of p105, the precursor form of p50 [  39].	transcription
57052	1	335335	7	NULL	NULL	0	NULL	ASMase			activate		may			 I B kinase complex					NULL		0	NULL	NULL	NULL	gw60_febslett_526_1_15_s_180	12208496	Hence, it is conceivable that ASMase may activate the I B kinase complex, which in turn leads to phosphorylation and proteasome-limited proteolysis of p105, the precursor form of p50 [  39].	transcription
57053	2	335335	7	NULL	NULL	0	NULL	statement 1			leads to					phosphorylation					NULL		0	NULL	NULL	NULL	gw60_febslett_526_1_15_s_180	12208496	Hence, it is conceivable that ASMase may activate the I B kinase complex, which in turn leads to phosphorylation and proteasome-limited proteolysis of p105, the precursor form of p50 [  39].	transcription
57054	3	335335	7	NULL	NULL	0	NULL	statement 1			leads to					p105		proteasome-limited proteolysis of 			NULL		0	NULL	NULL	NULL	gw60_febslett_526_1_15_s_180	12208496	Hence, it is conceivable that ASMase may activate the I B kinase complex, which in turn leads to phosphorylation and proteasome-limited proteolysis of p105, the precursor form of p50 [  39].	transcription
57055	4	335335	7	NULL	NULL	0	NULL	p105			is a precursor of					p50					NULL		0	NULL	NULL	NULL	gw60_febslett_526_1_15_s_180	12208496	Hence, it is conceivable that ASMase may activate the I B kinase complex, which in turn leads to phosphorylation and proteasome-limited proteolysis of p105, the precursor form of p50 [  39].	transcription
78198	1	335336	6	NULL	NULL	0	NULL	NF-B	GP		is a type of					Transcription factor	GP				NULL		0	NULL	NULL	NULL	gw60_febslett_529_1_22_s_62	12354607	The first example of this type of regulator was found in the p105 precursor of the transcription factor NF- B which contains a Gly rich region (GRR) that is required for processing to the active p50 [  17].	transcription
78199	2	335336	6	NULL	NULL	0	NULL	NF-B	GP		contains						AminoAcid		Gly rich region		NULL		0	NULL	NULL	NULL	gw60_febslett_529_1_22_s_62	12354607	The first example of this type of regulator was found in the p105 precursor of the transcription factor NF- B which contains a Gly rich region (GRR) that is required for processing to the active p50 [  17].	transcription
78200	3	335336	6	NULL	NULL	0	NULL	GRR	AminoAcid		is					Gly rich region	AminoAcid				NULL		0	NULL	NULL	NULL	gw60_febslett_529_1_22_s_62	12354607	The first example of this type of regulator was found in the p105 precursor of the transcription factor NF- B which contains a Gly rich region (GRR) that is required for processing to the active p50 [  17].	transcription
78201	4	335336	6	NULL	NULL	0	NULL	p105 precursor	GP		is processed to					p50	GP				NULL		0	NULL	NULL	NULL	gw60_febslett_529_1_22_s_62	12354607	The first example of this type of regulator was found in the p105 precursor of the transcription factor NF- B which contains a Gly rich region (GRR) that is required for processing to the active p50 [  17].	transcription
57056	1	335336	7	NULL	NULL	0	NULL	p105			is a precursor of					NF-B					NULL		0	NULL	NULL	NULL	gw60_febslett_529_1_22_s_62	12354607	The first example of this type of regulator was found in the p105 precursor of the transcription factor NF- B which contains a Gly rich region (GRR) that is required for processing to the active p50 [  17].	transcription
57057	2	335336	7	NULL	NULL	0	NULL	NF-B			is a type of					transcription factor					NULL		0	NULL	NULL	NULL	gw60_febslett_529_1_22_s_62	12354607	The first example of this type of regulator was found in the p105 precursor of the transcription factor NF- B which contains a Gly rich region (GRR) that is required for processing to the active p50 [  17].	transcription
57058	3	335336	7	NULL	NULL	0	NULL	NF-B			contains								Gly rich region (GRR)		NULL		0	NULL	NULL	NULL	gw60_febslett_529_1_22_s_62	12354607	The first example of this type of regulator was found in the p105 precursor of the transcription factor NF- B which contains a Gly rich region (GRR) that is required for processing to the active p50 [  17].	transcription
57059	4	335336	7	NULL	NULL	0	NULL	statement 3			is required for					p50		processing to active			NULL		0	NULL	NULL	NULL	gw60_febslett_529_1_22_s_62	12354607	The first example of this type of regulator was found in the p105 precursor of the transcription factor NF- B which contains a Gly rich region (GRR) that is required for processing to the active p50 [  17].	transcription
57060	1	335337	7	NULL	NULL	0	NULL	clasto-lactacystin beta-lactone			inhibits					p50		generation of			NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_152	9529257	The addition of  clasto-lactacystin beta-lactone at concentrations as low as 10  muM inhibited the generation of p50 while not altering the production of  p105 (  Figure 6, compare lanes 1 - 4 with lanes 5 - 8).	transcription
57061	2	335337	7	NULL	NULL	0	NULL	clasto-lactacystin beta-lactone			does not alter					p105		production of			NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_152	9529257	The addition of  clasto-lactacystin beta-lactone at concentrations as low as 10  muM inhibited the generation of p50 while not altering the production of  p105 (  Figure 6, compare lanes 1 - 4 with lanes 5 - 8).	transcription
57062	1	335338	7	NULL	NULL	0	NULL	Proteasome inhibitor			blocks					p50		Cotranslational Generation of			NULL		0	NULL	NULL	NULL	gw60_cell_92_6_819_s_155	9529257	Cotranslational Generation of p50 Is Blocked by a Specific  Inhibitor of the Proteasome CHO-CD14 cells were transfected with a p105 expression vector  containing an N-terminal gp 10 epitope tag.	transcription
57063	1	335339	7	NULL	NULL	0	NULL	Myc			bind					p50					NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_62	9950430	An anti-Myc monoclonal antibody caused a supershift of the induced smaller NF-kappaB complex in cells that had been co-transfected with TPL-2 and Myc - p105 (  Fig. 4c, lane 8), confirming the presence of Myc - p50 in this complex.	transcription
78202	1	335340	6	NULL	NULL	0	NULL	TNF-alpha	GP		stimulates					p105	GP	degradation of 			NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_89	9950430	In Jurkat T cells stably transfected with control vector, tumour-necrosis factor-alpha (TNF-alpha) stimulated p105 degradation ( Fig. 7a) while having no detectable effect on p50 production (data not shown).	transcription
78203	2	335340	6	NULL	NULL	0	NULL	TNF-alpha	GP		is					 tumour-necrosis factor-alpha	GP				NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_89	9950430	In Jurkat T cells stably transfected with control vector, tumour-necrosis factor-alpha (TNF-alpha) stimulated p105 degradation ( Fig. 7a) while having no detectable effect on p50 production (data not shown).	transcription
57064	1	335340	7	NULL	NULL	0	NULL	TNF-alpha			stimulates					p105		degradation of			NULL	Jurkat T cells	0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_89	9950430	In Jurkat T cells stably transfected with control vector, tumour-necrosis factor-alpha (TNF-alpha) stimulated p105 degradation ( Fig. 7a) while having no detectable effect on p50 production (data not shown).	transcription
57065	2	335340	7	NULL	NULL	0	NULL	TNF-alpha			is					tumour-necrosis factor-alpha					NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_89	9950430	In Jurkat T cells stably transfected with control vector, tumour-necrosis factor-alpha (TNF-alpha) stimulated p105 degradation ( Fig. 7a) while having no detectable effect on p50 production (data not shown).	transcription
57066	3	335340	7	NULL	NULL	0	NULL	TNF-alpha			does not effect					p50		production of			NULL		0	NULL	NULL	NULL	gw60_nature_397_6717_363_s_89	9950430	In Jurkat T cells stably transfected with control vector, tumour-necrosis factor-alpha (TNF-alpha) stimulated p105 degradation ( Fig. 7a) while having no detectable effect on p50 production (data not shown).	transcription
78204	1	335341	6	NULL	NULL	0	NULL	DA-IKK	GP		induces					p105	GP	loss of			NULL		0	NULL	NULL	NULL	gw60_molcell_7_2_401_s_105	11239468	Consistent with one recent report  (Heissmeyer et al., 1999  ), DA-IKK  induced significant loss of p105 without significantly enhancing the production of p50 (lane 2).	transcription
78205	2	335341	6	NULL	NULL	0	NULL	DA-IKK	GP		does not enhance					p50	GP	production of 			NULL		0	NULL	NULL	NULL	gw60_molcell_7_2_401_s_105	11239468	Consistent with one recent report  (Heissmeyer et al., 1999  ), DA-IKK  induced significant loss of p105 without significantly enhancing the production of p50 (lane 2).	transcription
57067	1	335341	7	NULL	NULL	0	NULL	DA-IKK			induce					p105		significant loss of 			NULL		0	NULL	NULL	NULL	gw60_molcell_7_2_401_s_105	11239468	Consistent with one recent report  (Heissmeyer et al., 1999  ), DA-IKK  induced significant loss of p105 without significantly enhancing the production of p50 (lane 2).	transcription
57068	2	335341	7	NULL	NULL	0	NULL	statement 1			does not enhance		significantly			p50		production of			NULL		0	NULL	NULL	NULL	gw60_molcell_7_2_401_s_105	11239468	Consistent with one recent report  (Heissmeyer et al., 1999  ), DA-IKK  induced significant loss of p105 without significantly enhancing the production of p50 (lane 2).	transcription
78206	1	335342	6	NULL	NULL	0	NULL	NFKB1	GP		encodes					p105	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_421	11158290	The complete exon-intron structure of the 156-kb human gene NFKB1, which encodes the p105 and p50 proteins of transcription factors NF-kappaB and IkappaBgamma: implications for NF-kappaB-mediated signal transduction.	transcription
78207	2	335342	6	NULL	NULL	0	NULL	NFKB1	GP		encodes					p50	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_421	11158290	The complete exon-intron structure of the 156-kb human gene NFKB1, which encodes the p105 and p50 proteins of transcription factors NF-kappaB and IkappaBgamma: implications for NF-kappaB-mediated signal transduction.	transcription
78208	3	335342	6	NULL	NULL	NULL	NULL	p105	GP		is a type of					Transcription factor	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_421	11158290	The complete exon-intron structure of the 156-kb human gene NFKB1, which encodes the p105 and p50 proteins of transcription factors NF-kappaB and IkappaBgamma: implications for NF-kappaB-mediated signal transduction.	transcription
78209	4	335342	6	NULL	NULL	0	NULL	p50	GP		is a type of					Transcription factor	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_421	11158290	The complete exon-intron structure of the 156-kb human gene NFKB1, which encodes the p105 and p50 proteins of transcription factors NF-kappaB and IkappaBgamma: implications for NF-kappaB-mediated signal transduction.	transcription
57069	1	335342	7	NULL	NULL	0	NULL	NFKB1 gene		human	encode					p105 protein					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_421	11158290	The complete exon-intron structure of the 156-kb human gene NFKB1, which encodes the p105 and p50 proteins of transcription factors NF-kappaB and IkappaBgamma: implications for NF-kappaB-mediated signal transduction.	transcription
57070	2	335342	7	NULL	NULL	0	NULL	NFKB1 gene		human	encode					p50 protein					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_421	11158290	The complete exon-intron structure of the 156-kb human gene NFKB1, which encodes the p105 and p50 proteins of transcription factors NF-kappaB and IkappaBgamma: implications for NF-kappaB-mediated signal transduction.	transcription
57071	3	335342	7	NULL	NULL	0	NULL	NF-kappaB 			is a type of					transcription factor					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_421	11158290	The complete exon-intron structure of the 156-kb human gene NFKB1, which encodes the p105 and p50 proteins of transcription factors NF-kappaB and IkappaBgamma: implications for NF-kappaB-mediated signal transduction.	transcription
57072	4	335342	7	NULL	NULL	0	NULL	IkappaBgamma			is a type of					transcription factor					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1024_s_421	11158290	The complete exon-intron structure of the 156-kb human gene NFKB1, which encodes the p105 and p50 proteins of transcription factors NF-kappaB and IkappaBgamma: implications for NF-kappaB-mediated signal transduction.	transcription
78210	1	335344	6	NULL	NULL	0	NULL	p105 molecule	GP		contain								ankyrin repeats		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_5	11350967	Here we show that processing of p105 molecules that contain more then four ankyrin repeats, but lack the C-terminal phosphorylation/ubiquitin ligase binding domain, is strongly inhibited by docked p50 subunits.	transcription
78211	2	335344	6	NULL	NULL	0	NULL	p105 molecule	GP		lack								 C-terminal phosphorylation/ubiquitin ligase binding domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_5	11350967	Here we show that processing of p105 molecules that contain more then four ankyrin repeats, but lack the C-terminal phosphorylation/ubiquitin ligase binding domain, is strongly inhibited by docked p50 subunits.	transcription
78212	3	335344	6	NULL	NULL	0	NULL	p105 molecule 	GP	processing of	is inhibited by		strongly			p50 subunit	GP	docked			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_5	11350967	Here we show that processing of p105 molecules that contain more then four ankyrin repeats, but lack the C-terminal phosphorylation/ubiquitin ligase binding domain, is strongly inhibited by docked p50 subunits.	transcription
57073	1	335344	7	NULL	NULL	0	NULL	p105 molecules			contain								four ankyrin repeats		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_5	11350967	Here we show that processing of p105 molecules that contain more then four ankyrin repeats, but lack the C-terminal phosphorylation/ubiquitin ligase binding domain, is strongly inhibited by docked p50 subunits.	transcription
57074	2	335344	7	NULL	NULL	0	NULL	p105 molecules			lack								C-terminal phosphorylation/ubiquitin ligase binding domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_5	11350967	Here we show that processing of p105 molecules that contain more then four ankyrin repeats, but lack the C-terminal phosphorylation/ubiquitin ligase binding domain, is strongly inhibited by docked p50 subunits.	transcription
57075	3	335344	7	NULL	NULL	0	NULL	statement 1			occur simulataneous with					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_5	11350967	Here we show that processing of p105 molecules that contain more then four ankyrin repeats, but lack the C-terminal phosphorylation/ubiquitin ligase binding domain, is strongly inhibited by docked p50 subunits.	transcription
57076	4	335344	7	NULL	NULL	0	NULL			docked	inhibits		strongly	p50 subunits		statement 3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_5	11350967	Here we show that processing of p105 molecules that contain more then four ankyrin repeats, but lack the C-terminal phosphorylation/ubiquitin ligase binding domain, is strongly inhibited by docked p50 subunits.	transcription
57077	1	335345	7	NULL	NULL	0	NULL	p105 			contain							more than	four ankyrin repeats		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_147	11350967	Exogenous p50 inhibits  in vitro processing of p105 species that contain more than four ankyrin repeats but lack the C-terminal  IKK  phosphorylation and beta-TrCP binding domain.	transcription
57078	2	335345	7	NULL	NULL	0	NULL	p105			lack								C-terminal IKK phosphorylation domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_147	11350967	Exogenous p50 inhibits  in vitro processing of p105 species that contain more than four ankyrin repeats but lack the C-terminal  IKK  phosphorylation and beta-TrCP binding domain.	transcription
57079	3	335345	7	NULL	NULL	0	NULL	p105			lack								beta-TrCP binding domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_147	11350967	Exogenous p50 inhibits  in vitro processing of p105 species that contain more than four ankyrin repeats but lack the C-terminal  IKK  phosphorylation and beta-TrCP binding domain.	transcription
57080	4	335345	7	NULL	NULL	0	NULL	statement 1			occur simulataneous with					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_147	11350967	Exogenous p50 inhibits  in vitro processing of p105 species that contain more than four ankyrin repeats but lack the C-terminal  IKK  phosphorylation and beta-TrCP binding domain.	transcription
57081	5	335345	7	NULL	NULL	0	NULL	statement 2			occur simulataneous with					statement 3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_147	11350967	Exogenous p50 inhibits  in vitro processing of p105 species that contain more than four ankyrin repeats but lack the C-terminal  IKK  phosphorylation and beta-TrCP binding domain.	transcription
57082	6	335345	7	NULL	NULL	0	NULL	p50		exogenous	inhibits					statement 4		processing of			NULL	in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_147	11350967	Exogenous p50 inhibits  in vitro processing of p105 species that contain more than four ankyrin repeats but lack the C-terminal  IKK  phosphorylation and beta-TrCP binding domain.	transcription
57083	7	335345	7	NULL	NULL	0	NULL	p50		exogenous	inhibits					statement 5		processing of			NULL	in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_147	11350967	Exogenous p50 inhibits  in vitro processing of p105 species that contain more than four ankyrin repeats but lack the C-terminal  IKK  phosphorylation and beta-TrCP binding domain.	transcription
78730	1	335346	6	NULL	NULL	0	NULL	mice	Organism		express					p50	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_34_31479_s_13	12807880	However, mice expressing  p50 but lacking p105 suffer severe defects that include lymphocyte  infiltration in multiple organs and a lack of normal cytokine expression in  macrophages, leading to their high postnatal fatality  ( 5).	transcription
78731	2	335346	6	NULL	NULL	0	NULL	mice	Organism		lack					p105	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_34_31479_s_13	12807880	However, mice expressing  p50 but lacking p105 suffer severe defects that include lymphocyte  infiltration in multiple organs and a lack of normal cytokine expression in  macrophages, leading to their high postnatal fatality  ( 5).	transcription
78732	3	335346	6	NULL	NULL	0	NULL	statement 1	Process		occurs simultaneously with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_34_31479_s_13	12807880	However, mice expressing  p50 but lacking p105 suffer severe defects that include lymphocyte  infiltration in multiple organs and a lack of normal cytokine expression in  macrophages, leading to their high postnatal fatality  ( 5).	transcription
78733	4	335346	6	NULL	NULL	0	NULL	statement 3	Process		leads to					lymphocyte infiltration	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_34_31479_s_13	12807880	However, mice expressing  p50 but lacking p105 suffer severe defects that include lymphocyte  infiltration in multiple organs and a lack of normal cytokine expression in  macrophages, leading to their high postnatal fatality  ( 5).	transcription
78734	5	335346	6	NULL	NULL	0	NULL	cytokine	Chemical		is expressed in					macrophages	Cell				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_34_31479_s_13	12807880	However, mice expressing  p50 but lacking p105 suffer severe defects that include lymphocyte  infiltration in multiple organs and a lack of normal cytokine expression in  macrophages, leading to their high postnatal fatality  ( 5).	transcription
78735	6	335346	6	NULL	NULL	0	NULL	statement 3	Process		causes					statement 5	Process	lack of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_34_31479_s_13	12807880	However, mice expressing  p50 but lacking p105 suffer severe defects that include lymphocyte  infiltration in multiple organs and a lack of normal cytokine expression in  macrophages, leading to their high postnatal fatality  ( 5).	transcription
57084	1	335346	7	NULL	NULL	0	NULL	mice 			express					p50					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_34_31479_s_13	12807880	However, mice expressing  p50 but lacking p105 suffer severe defects that include lymphocyte  infiltration in multiple organs and a lack of normal cytokine expression in  macrophages, leading to their high postnatal fatality  ( 5).	transcription
57085	2	335346	7	NULL	NULL	0	NULL	statement 1			lacks					p105					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_34_31479_s_13	12807880	However, mice expressing  p50 but lacking p105 suffer severe defects that include lymphocyte  infiltration in multiple organs and a lack of normal cytokine expression in  macrophages, leading to their high postnatal fatality  ( 5).	transcription
57086	3	335346	7	NULL	NULL	0	NULL	statement 2			suffer from					lymphocyte infiltration					NULL	multiple organs	0	NULL	NULL	NULL	gw60_jbiolchem_278_34_31479_s_13	12807880	However, mice expressing  p50 but lacking p105 suffer severe defects that include lymphocyte  infiltration in multiple organs and a lack of normal cytokine expression in  macrophages, leading to their high postnatal fatality  ( 5).	transcription
57087	4	335346	7	NULL	NULL	0	NULL	statement 2			leads to					cytokine		 lack of normal expression of			NULL	macrophages	0	NULL	NULL	NULL	gw60_jbiolchem_278_34_31479_s_13	12807880	However, mice expressing  p50 but lacking p105 suffer severe defects that include lymphocyte  infiltration in multiple organs and a lack of normal cytokine expression in  macrophages, leading to their high postnatal fatality  ( 5).	transcription
57088	5	335346	7	NULL	NULL	0	NULL	statement 3			leads to					high postnatal fatality					NULL	mice	NULL	NULL	NULL	NULL	gw60_jbiolchem_278_34_31479_s_13	12807880	However, mice expressing  p50 but lacking p105 suffer severe defects that include lymphocyte  infiltration in multiple organs and a lack of normal cytokine expression in  macrophages, leading to their high postnatal fatality  ( 5).	transcription
57089	6	335346	7	NULL	NULL	0	NULL	statement 4			leads to					high postnatal fatality					NULL	mice	0	NULL	NULL	NULL	gw60_jbiolchem_278_34_31479_s_13	12807880	However, mice expressing  p50 but lacking p105 suffer severe defects that include lymphocyte  infiltration in multiple organs and a lack of normal cytokine expression in  macrophages, leading to their high postnatal fatality  ( 5).	transcription
78213	1	335348	6	NULL	NULL	0	NULL	PMA	Chemical		activates					NF-kappaB	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31244_s_94	8537390	In concomitance with NF-kappaB  activation by PMA, the processing of p105 did not occur in the nucleus ( Fig. 3,  B  and  C), and the nuclear content of  p50 was unchanged ( Fig. 3 B).	transcription
57090	1	335348	7	NULL	NULL	0	NULL	PMA			activates					NF-kappaB					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31244_s_94	8537390	In concomitance with NF-kappaB  activation by PMA, the processing of p105 did not occur in the nucleus ( Fig. 3,  B  and  C), and the nuclear content of  p50 was unchanged ( Fig. 3 B).	transcription
57091	2	335348	7	NULL	NULL	0	NULL	p105		processing of	does not occur in					nucleus					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31244_s_94	8537390	In concomitance with NF-kappaB  activation by PMA, the processing of p105 did not occur in the nucleus ( Fig. 3,  B  and  C), and the nuclear content of  p50 was unchanged ( Fig. 3 B).	transcription
57092	3	335348	7	NULL	NULL	0	NULL	p50		nuclear content of	remains					unchanged					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31244_s_94	8537390	In concomitance with NF-kappaB  activation by PMA, the processing of p105 did not occur in the nucleus ( Fig. 3,  B  and  C), and the nuclear content of  p50 was unchanged ( Fig. 3 B).	transcription
57093	4	335348	7	NULL	NULL	0	NULL	statement 2			in concomitance with					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31244_s_94	8537390	In concomitance with NF-kappaB  activation by PMA, the processing of p105 did not occur in the nucleus ( Fig. 3,  B  and  C), and the nuclear content of  p50 was unchanged ( Fig. 3 B).	transcription
57094	5	335348	7	NULL	NULL	0	NULL	statement 3			in concomitance with					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_52_31244_s_94	8537390	In concomitance with NF-kappaB  activation by PMA, the processing of p105 did not occur in the nucleus ( Fig. 3,  B  and  C), and the nuclear content of  p50 was unchanged ( Fig. 3 B).	transcription
78214	1	335349	6	NULL	NULL	0	NULL	p105	GP		is processed to					p50	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_21	7814425	Here we demonstrate that treatment of human monocytic cells with either  bacterial lipopolysaccharide (LPS) or tumor necrosis factor-alpha  (TNF)  stimulates p105 processing to p50 via an ATP-dependent pathway.	transcription
78215	2	335349	6	NULL	NULL	0	NULL	statement 1	process		is dependent on					ATP	process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_21	7814425	Here we demonstrate that treatment of human monocytic cells with either  bacterial lipopolysaccharide (LPS) or tumor necrosis factor-alpha  (TNF)  stimulates p105 processing to p50 via an ATP-dependent pathway.	transcription
78216	3	335349	6	NULL	NULL	0	NULL	LPS	Chemical		stimulates					statement 1	process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_21	7814425	Here we demonstrate that treatment of human monocytic cells with either  bacterial lipopolysaccharide (LPS) or tumor necrosis factor-alpha  (TNF)  stimulates p105 processing to p50 via an ATP-dependent pathway.	transcription
78217	4	335349	6	NULL	NULL	0	NULL	TNF	Chemical		stimulates					statement 1	process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_21	7814425	Here we demonstrate that treatment of human monocytic cells with either  bacterial lipopolysaccharide (LPS) or tumor necrosis factor-alpha  (TNF)  stimulates p105 processing to p50 via an ATP-dependent pathway.	transcription
57095	1	335349	7	NULL	NULL	0	NULL	p105			processed to					p50					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_21	7814425	Here we demonstrate that treatment of human monocytic cells with either  bacterial lipopolysaccharide (LPS) or tumor necrosis factor-alpha  (TNF)  stimulates p105 processing to p50 via an ATP-dependent pathway.	transcription
57096	2	335349	7	NULL	NULL	0	NULL	LPS			stimulates					statement 1					NULL	human monocytic cells	0	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_21	7814425	Here we demonstrate that treatment of human monocytic cells with either  bacterial lipopolysaccharide (LPS) or tumor necrosis factor-alpha  (TNF)  stimulates p105 processing to p50 via an ATP-dependent pathway.	transcription
57097	3	335349	7	NULL	NULL	0	NULL	TNF-alpha			stimulates					statement 1					NULL	human monocytic cells	0	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_21	7814425	Here we demonstrate that treatment of human monocytic cells with either  bacterial lipopolysaccharide (LPS) or tumor necrosis factor-alpha  (TNF)  stimulates p105 processing to p50 via an ATP-dependent pathway.	transcription
57098	4	335349	7	NULL	NULL	0	NULL	statement 1			via an					ATP-dependent pathway					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_21	7814425	Here we demonstrate that treatment of human monocytic cells with either  bacterial lipopolysaccharide (LPS) or tumor necrosis factor-alpha  (TNF)  stimulates p105 processing to p50 via an ATP-dependent pathway.	transcription
57099	5	335349	7	NULL	NULL	0	NULL	LPS			is					bacterial lipopolysaccharide					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_21	7814425	Here we demonstrate that treatment of human monocytic cells with either  bacterial lipopolysaccharide (LPS) or tumor necrosis factor-alpha  (TNF)  stimulates p105 processing to p50 via an ATP-dependent pathway.	transcription
57100	6	335349	7	NULL	NULL	0	NULL	TNF			is					tumor necrosis factor					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_21	7814425	Here we demonstrate that treatment of human monocytic cells with either  bacterial lipopolysaccharide (LPS) or tumor necrosis factor-alpha  (TNF)  stimulates p105 processing to p50 via an ATP-dependent pathway.	transcription
57101	7	335349	7	NULL	NULL	0	NULL	statement 2			is an alternative to					statement 3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_21	7814425	Here we demonstrate that treatment of human monocytic cells with either  bacterial lipopolysaccharide (LPS) or tumor necrosis factor-alpha  (TNF)  stimulates p105 processing to p50 via an ATP-dependent pathway.	transcription
57102	1	335350	7	NULL	NULL	0	NULL	p105			forms					p50					NULL		0	NULL	NULL	NULL	abs-batch0740-0759_febs-j_273_16_16911524_s_10	16911524	Western blot analysis revealed transient activation of p38 mitogen-activated  protein kinase, extracellular signal-related kinase 1/2, and nuclear factor  kappaB1 and possibly new formation of p50 from its precursor p105.	transcription
57103	2	335350	7	NULL	NULL	0	NULL	p105			is a precursor of					p50					NULL		0	NULL	NULL	NULL	abs-batch0740-0759_febs-j_273_16_16911524_s_10	16911524	Western blot analysis revealed transient activation of p38 mitogen-activated  protein kinase, extracellular signal-related kinase 1/2, and nuclear factor  kappaB1 and possibly new formation of p50 from its precursor p105.	transcription
78218	1	335351	6	NULL	NULL	0	NULL	TNF-alpha	GP		activates					PI3K/Akt	GP				NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_282	16192643	Activation of PI3K/Akt by the cytokine TNF-alpha or other factors, induces the phosphorylation and inactivation of GSK-3beta in neurons,  which in turn 1) impairs nuclear import of p65, 2) decreases the processing of p105  to p50, and 3) reduces proteasome (prot)-mediated degradation of p50.	transcription
78219	2	335351	6	NULL	NULL	0	NULL	TNF-alpha	GP		is a type of					cytokine	GP				NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_282	16192643	Activation of PI3K/Akt by the cytokine TNF-alpha or other factors, induces the phosphorylation and inactivation of GSK-3beta in neurons,  which in turn 1) impairs nuclear import of p65, 2) decreases the processing of p105  to p50, and 3) reduces proteasome (prot)-mediated degradation of p50.	transcription
78220	3	335351	6	NULL	NULL	NULL	NULL	statement 1	process		induces					GSK-3beta	GP	phosphorylation of			NULL	neurons	NULL	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_282	16192643	Activation of PI3K/Akt by the cytokine TNF-alpha or other factors, induces the phosphorylation and inactivation of GSK-3beta in neurons,  which in turn 1) impairs nuclear import of p65, 2) decreases the processing of p105  to p50, and 3) reduces proteasome (prot)-mediated degradation of p50.	transcription
78221	4	335351	6	NULL	NULL	0	NULL	statement 1	process		induces					GSK-3beta	GP	inactivation of			NULL	neurons	0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_282	16192643	Activation of PI3K/Akt by the cytokine TNF-alpha or other factors, induces the phosphorylation and inactivation of GSK-3beta in neurons,  which in turn 1) impairs nuclear import of p65, 2) decreases the processing of p105  to p50, and 3) reduces proteasome (prot)-mediated degradation of p50.	transcription
78222	5	335351	6	NULL	NULL	0	NULL	p65	GP		is imported to					nucleus	CellComponent				NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_282	16192643	Activation of PI3K/Akt by the cytokine TNF-alpha or other factors, induces the phosphorylation and inactivation of GSK-3beta in neurons,  which in turn 1) impairs nuclear import of p65, 2) decreases the processing of p105  to p50, and 3) reduces proteasome (prot)-mediated degradation of p50.	transcription
78223	6	335351	6	NULL	NULL	0	NULL	statement 3	process		impairs					statement 5	process				NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_282	16192643	Activation of PI3K/Akt by the cytokine TNF-alpha or other factors, induces the phosphorylation and inactivation of GSK-3beta in neurons,  which in turn 1) impairs nuclear import of p65, 2) decreases the processing of p105  to p50, and 3) reduces proteasome (prot)-mediated degradation of p50.	transcription
78224	7	335351	6	NULL	NULL	0	NULL	p50	GP		is processed to					p105	GP				NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_282	16192643	Activation of PI3K/Akt by the cytokine TNF-alpha or other factors, induces the phosphorylation and inactivation of GSK-3beta in neurons,  which in turn 1) impairs nuclear import of p65, 2) decreases the processing of p105  to p50, and 3) reduces proteasome (prot)-mediated degradation of p50.	transcription
78225	8	335351	6	NULL	NULL	0	NULL	statement 3	process		decreases					statement 7	process				NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_282	16192643	Activation of PI3K/Akt by the cytokine TNF-alpha or other factors, induces the phosphorylation and inactivation of GSK-3beta in neurons,  which in turn 1) impairs nuclear import of p65, 2) decreases the processing of p105  to p50, and 3) reduces proteasome (prot)-mediated degradation of p50.	transcription
78226	9	335351	6	NULL	NULL	0	NULL	proteasome	CellComponent		mediates					p50	GP	degradation of 			NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_282	16192643	Activation of PI3K/Akt by the cytokine TNF-alpha or other factors, induces the phosphorylation and inactivation of GSK-3beta in neurons,  which in turn 1) impairs nuclear import of p65, 2) decreases the processing of p105  to p50, and 3) reduces proteasome (prot)-mediated degradation of p50.	transcription
78227	10	335351	6	NULL	NULL	0	NULL	statement 3	process		reduces					statement 9	process				NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_282	16192643	Activation of PI3K/Akt by the cytokine TNF-alpha or other factors, induces the phosphorylation and inactivation of GSK-3beta in neurons,  which in turn 1) impairs nuclear import of p65, 2) decreases the processing of p105  to p50, and 3) reduces proteasome (prot)-mediated degradation of p50.	transcription
57106	1	335351	7	NULL	NULL	0	NULL	TNF-alpha			activates					PI3K/Akt 					NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_282	16192643	Activation of PI3K/Akt by the cytokine TNF-alpha or other factors, induces the phosphorylation and inactivation of GSK-3beta in neurons,  which in turn 1) impairs nuclear import of p65, 2) decreases the processing of p105  to p50, and 3) reduces proteasome (prot)-mediated degradation of p50.	transcription
57107	2	335351	7	NULL	NULL	0	NULL	statement 1			induces					GSK-3beta 		phosphorylation of			NULL	neurons	0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_282	16192643	Activation of PI3K/Akt by the cytokine TNF-alpha or other factors, induces the phosphorylation and inactivation of GSK-3beta in neurons,  which in turn 1) impairs nuclear import of p65, 2) decreases the processing of p105  to p50, and 3) reduces proteasome (prot)-mediated degradation of p50.	transcription
57108	3	335351	7	NULL	NULL	0	NULL	statement 1			induces					GSK-3beta 		inactivation of			NULL	neurons	0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_282	16192643	Activation of PI3K/Akt by the cytokine TNF-alpha or other factors, induces the phosphorylation and inactivation of GSK-3beta in neurons,  which in turn 1) impairs nuclear import of p65, 2) decreases the processing of p105  to p50, and 3) reduces proteasome (prot)-mediated degradation of p50.	transcription
57109	4	335351	7	NULL	NULL	0	NULL	statement 2			occur simulataneous with					statement 3					NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_282	16192643	Activation of PI3K/Akt by the cytokine TNF-alpha or other factors, induces the phosphorylation and inactivation of GSK-3beta in neurons,  which in turn 1) impairs nuclear import of p65, 2) decreases the processing of p105  to p50, and 3) reduces proteasome (prot)-mediated degradation of p50.	transcription
57110	5	335351	7	NULL	NULL	0	NULL	statement 4			impairs					p65		nuclear import of 			NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_282	16192643	Activation of PI3K/Akt by the cytokine TNF-alpha or other factors, induces the phosphorylation and inactivation of GSK-3beta in neurons,  which in turn 1) impairs nuclear import of p65, 2) decreases the processing of p105  to p50, and 3) reduces proteasome (prot)-mediated degradation of p50.	transcription
57111	6	335351	7	NULL	NULL	0	NULL	p150			processed to					p50					NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_282	16192643	Activation of PI3K/Akt by the cytokine TNF-alpha or other factors, induces the phosphorylation and inactivation of GSK-3beta in neurons,  which in turn 1) impairs nuclear import of p65, 2) decreases the processing of p105  to p50, and 3) reduces proteasome (prot)-mediated degradation of p50.	transcription
57112	7	335351	7	NULL	NULL	0	NULL	statement 4			decreases					statement 6					NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_282	16192643	Activation of PI3K/Akt by the cytokine TNF-alpha or other factors, induces the phosphorylation and inactivation of GSK-3beta in neurons,  which in turn 1) impairs nuclear import of p65, 2) decreases the processing of p105  to p50, and 3) reduces proteasome (prot)-mediated degradation of p50.	transcription
57113	8	335351	7	NULL	NULL	0	NULL	proteasome			mediate					p50		degradation of			NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_282	16192643	Activation of PI3K/Akt by the cytokine TNF-alpha or other factors, induces the phosphorylation and inactivation of GSK-3beta in neurons,  which in turn 1) impairs nuclear import of p65, 2) decreases the processing of p105  to p50, and 3) reduces proteasome (prot)-mediated degradation of p50.	transcription
57114	9	335351	7	NULL	NULL	0	NULL	statement 4			reduces					statement 6					NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_282	16192643	Activation of PI3K/Akt by the cytokine TNF-alpha or other factors, induces the phosphorylation and inactivation of GSK-3beta in neurons,  which in turn 1) impairs nuclear import of p65, 2) decreases the processing of p105  to p50, and 3) reduces proteasome (prot)-mediated degradation of p50.	transcription
57115	10	335351	7	NULL	NULL	0	NULL	TNF-alpha			is a type of					cytokine					NULL		0	NULL	NULL	NULL	gw70_amjpathol_167_4_1081_s_282	16192643	Activation of PI3K/Akt by the cytokine TNF-alpha or other factors, induces the phosphorylation and inactivation of GSK-3beta in neurons,  which in turn 1) impairs nuclear import of p65, 2) decreases the processing of p105  to p50, and 3) reduces proteasome (prot)-mediated degradation of p50.	transcription
78228	1	335352	6	NULL	NULL	0	NULL	p100	GP		processed into					p52	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_2_1217_s_11	15536066	Limited proteolytic processing of the p100 and p105 proteins generates p52 and p50, respectively, and NF-kappaB DNA binding and transactivation is carried out by heterodimers of p50 or p52 with one of the transactivation-domain containing Rel proteins (RelA, RelB, or c-Rel) ( ).	transcription
78229	2	335352	6	NULL	NULL	0	NULL	p105	GP		processed into					p50	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_2_1217_s_11	15536066	Limited proteolytic processing of the p100 and p105 proteins generates p52 and p50, respectively, and NF-kappaB DNA binding and transactivation is carried out by heterodimers of p50 or p52 with one of the transactivation-domain containing Rel proteins (RelA, RelB, or c-Rel) ( ).	transcription
78230	3	335352	6	NULL	NULL	0	NULL	NF-kappaB	GP		bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_2_1217_s_11	15536066	Limited proteolytic processing of the p100 and p105 proteins generates p52 and p50, respectively, and NF-kappaB DNA binding and transactivation is carried out by heterodimers of p50 or p52 with one of the transactivation-domain containing Rel proteins (RelA, RelB, or c-Rel) ( ).	transcription
78231	4	335352	6	NULL	NULL	NULL	NULL	p50	GP		bind					RelA	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_2_1217_s_11	15536066	Limited proteolytic processing of the p100 and p105 proteins generates p52 and p50, respectively, and NF-kappaB DNA binding and transactivation is carried out by heterodimers of p50 or p52 with one of the transactivation-domain containing Rel proteins (RelA, RelB, or c-Rel) ( ).	transcription
78232	5	335352	6	NULL	NULL	0	NULL	p50	GP		bind					RelB	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_2_1217_s_11	15536066	Limited proteolytic processing of the p100 and p105 proteins generates p52 and p50, respectively, and NF-kappaB DNA binding and transactivation is carried out by heterodimers of p50 or p52 with one of the transactivation-domain containing Rel proteins (RelA, RelB, or c-Rel) ( ).	transcription
78233	6	335352	6	NULL	NULL	0	NULL	p50	GP		bind					c-Rel	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_2_1217_s_11	15536066	Limited proteolytic processing of the p100 and p105 proteins generates p52 and p50, respectively, and NF-kappaB DNA binding and transactivation is carried out by heterodimers of p50 or p52 with one of the transactivation-domain containing Rel proteins (RelA, RelB, or c-Rel) ( ).	transcription
78234	7	335352	6	NULL	NULL	0	NULL	p52	GP		bind					RelA	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_2_1217_s_11	15536066	Limited proteolytic processing of the p100 and p105 proteins generates p52 and p50, respectively, and NF-kappaB DNA binding and transactivation is carried out by heterodimers of p50 or p52 with one of the transactivation-domain containing Rel proteins (RelA, RelB, or c-Rel) ( ).	transcription
78235	8	335352	6	NULL	NULL	0	NULL	p52	GP		bind					RelB	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_2_1217_s_11	15536066	Limited proteolytic processing of the p100 and p105 proteins generates p52 and p50, respectively, and NF-kappaB DNA binding and transactivation is carried out by heterodimers of p50 or p52 with one of the transactivation-domain containing Rel proteins (RelA, RelB, or c-Rel) ( ).	transcription
78236	9	335352	6	NULL	NULL	0	NULL	p52	GP		bind					c-Rel	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_2_1217_s_11	15536066	Limited proteolytic processing of the p100 and p105 proteins generates p52 and p50, respectively, and NF-kappaB DNA binding and transactivation is carried out by heterodimers of p50 or p52 with one of the transactivation-domain containing Rel proteins (RelA, RelB, or c-Rel) ( ).	transcription
57116	1	335352	7	NULL	NULL	0	NULL	p100			proteolyse		limited			p52					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_2_1217_s_11	15536066	Limited proteolytic processing of the p100 and p105 proteins generates p52 and p50, respectively, and NF-kappaB DNA binding and transactivation is carried out by heterodimers of p50 or p52 with one of the transactivation-domain containing Rel proteins (RelA, RelB, or c-Rel) ( ).	transcription
57117	2	335352	7	NULL	NULL	0	NULL	p105			proteolyse		limited			p50					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_2_1217_s_11	15536066	Limited proteolytic processing of the p100 and p105 proteins generates p52 and p50, respectively, and NF-kappaB DNA binding and transactivation is carried out by heterodimers of p50 or p52 with one of the transactivation-domain containing Rel proteins (RelA, RelB, or c-Rel) ( ).	transcription
57118	3	335352	7	NULL	NULL	0	NULL	NF-kappaB			bind					DNA					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_2_1217_s_11	15536066	Limited proteolytic processing of the p100 and p105 proteins generates p52 and p50, respectively, and NF-kappaB DNA binding and transactivation is carried out by heterodimers of p50 or p52 with one of the transactivation-domain containing Rel proteins (RelA, RelB, or c-Rel) ( ).	transcription
57119	4	335352	7	NULL	NULL	0	NULL	p50 heterodimer			carries out					statement 3					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_2_1217_s_11	15536066	Limited proteolytic processing of the p100 and p105 proteins generates p52 and p50, respectively, and NF-kappaB DNA binding and transactivation is carried out by heterodimers of p50 or p52 with one of the transactivation-domain containing Rel proteins (RelA, RelB, or c-Rel) ( ).	transcription
57120	5	335352	7	NULL	NULL	0	NULL	p52			carries out					NF-kappaB		transactivation of	transactivation-domain containing RelA		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_2_1217_s_11	15536066	Limited proteolytic processing of the p100 and p105 proteins generates p52 and p50, respectively, and NF-kappaB DNA binding and transactivation is carried out by heterodimers of p50 or p52 with one of the transactivation-domain containing Rel proteins (RelA, RelB, or c-Rel) ( ).	transcription
57121	6	335352	7	NULL	NULL	0	NULL	p52			carries out					NF-kappaB		transactivation of	transactivation-domain containing RelB		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_2_1217_s_11	15536066	Limited proteolytic processing of the p100 and p105 proteins generates p52 and p50, respectively, and NF-kappaB DNA binding and transactivation is carried out by heterodimers of p50 or p52 with one of the transactivation-domain containing Rel proteins (RelA, RelB, or c-Rel) ( ).	transcription
57122	7	335352	7	NULL	NULL	0	NULL	p52			carries out					NF-kappaB		transactivation of	transactivation-domain containing c-Rel		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_2_1217_s_11	15536066	Limited proteolytic processing of the p100 and p105 proteins generates p52 and p50, respectively, and NF-kappaB DNA binding and transactivation is carried out by heterodimers of p50 or p52 with one of the transactivation-domain containing Rel proteins (RelA, RelB, or c-Rel) ( ).	transcription
57123	8	335352	7	NULL	NULL	0	NULL	p50 heterodimer			carries out					NF-kappaB		transactivation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_2_1217_s_11	15536066	Limited proteolytic processing of the p100 and p105 proteins generates p52 and p50, respectively, and NF-kappaB DNA binding and transactivation is carried out by heterodimers of p50 or p52 with one of the transactivation-domain containing Rel proteins (RelA, RelB, or c-Rel) ( ).	transcription
78724	1	335353	6	NULL	NULL	NULL	NULL	p105	GP	cleavage of	results in					RelB	GP				NULL		NULL	NULL	NULL	NULL	gw60_neurobiolaging_23_5_899_s_14	12392794	Unlike p65, RelB and c-Rel, the p50 and p49 subunits result from proteolytic cleavage of their p105 and p100 precursor molecules, respectively, which include C-terminal I B-like ankyrin repeats that inhibit p50 and p49 activity.	transcription
78725	2	335353	6	NULL	NULL	0	NULL	p105	GP	cleavage of	results in					c-Rel	GP				NULL		0	NULL	NULL	NULL	gw60_neurobiolaging_23_5_899_s_14	12392794	Unlike p65, RelB and c-Rel, the p50 and p49 subunits result from proteolytic cleavage of their p105 and p100 precursor molecules, respectively, which include C-terminal I B-like ankyrin repeats that inhibit p50 and p49 activity.	transcription
78726	3	335353	6	NULL	NULL	0	NULL	p100	GP	cleavage of	results in					p50	GP				NULL		0	NULL	NULL	NULL	gw60_neurobiolaging_23_5_899_s_14	12392794	Unlike p65, RelB and c-Rel, the p50 and p49 subunits result from proteolytic cleavage of their p105 and p100 precursor molecules, respectively, which include C-terminal I B-like ankyrin repeats that inhibit p50 and p49 activity.	transcription
78727	4	335353	6	NULL	NULL	0	NULL	p100	GP	cleavage of	results in					p49	GP				NULL		0	NULL	NULL	NULL	gw60_neurobiolaging_23_5_899_s_14	12392794	Unlike p65, RelB and c-Rel, the p50 and p49 subunits result from proteolytic cleavage of their p105 and p100 precursor molecules, respectively, which include C-terminal I B-like ankyrin repeats that inhibit p50 and p49 activity.	transcription
78728	5	335353	6	NULL	NULL	0	NULL				inhibits			C-terminal I B-like ankyrin repeat		p50	GP	activity of			NULL		0	NULL	NULL	NULL	gw60_neurobiolaging_23_5_899_s_14	12392794	Unlike p65, RelB and c-Rel, the p50 and p49 subunits result from proteolytic cleavage of their p105 and p100 precursor molecules, respectively, which include C-terminal I B-like ankyrin repeats that inhibit p50 and p49 activity.	transcription
78729	6	335353	6	NULL	NULL	0	NULL				inhibits			C-terminal I B-like ankyrin repeat		p49	GP	activity of			NULL		0	NULL	NULL	NULL	gw60_neurobiolaging_23_5_899_s_14	12392794	Unlike p65, RelB and c-Rel, the p50 and p49 subunits result from proteolytic cleavage of their p105 and p100 precursor molecules, respectively, which include C-terminal I B-like ankyrin repeats that inhibit p50 and p49 activity.	transcription
57126	1	335353	7	NULL	NULL	0	NULL				result from			p50 subunits		p105 precursor molecules		proteolytic cleavage of			NULL		0	NULL	NULL	NULL	gw60_neurobiolaging_23_5_899_s_14	12392794	Unlike p65, RelB and c-Rel, the p50 and p49 subunits result from proteolytic cleavage of their p105 and p100 precursor molecules, respectively, which include C-terminal I B-like ankyrin repeats that inhibit p50 and p49 activity.	transcription
57127	2	335353	7	NULL	NULL	0	NULL				result from			p49 subunits		p100 precursor molecules		proteolytic cleavage of			NULL		0	NULL	NULL	NULL	gw60_neurobiolaging_23_5_899_s_14	12392794	Unlike p65, RelB and c-Rel, the p50 and p49 subunits result from proteolytic cleavage of their p105 and p100 precursor molecules, respectively, which include C-terminal I B-like ankyrin repeats that inhibit p50 and p49 activity.	transcription
57128	3	335353	7	NULL	NULL	0	NULL	p105 precursor molecule			include								C-terminal I B-like ankyrin repeats		NULL		NULL	NULL	NULL	NULL	gw60_neurobiolaging_23_5_899_s_14	12392794	Unlike p65, RelB and c-Rel, the p50 and p49 subunits result from proteolytic cleavage of their p105 and p100 precursor molecules, respectively, which include C-terminal I B-like ankyrin repeats that inhibit p50 and p49 activity.	transcription
57129	4	335353	7	NULL	NULL	0	NULL	p100 precursor molecule			include								C-terminal I B-like ankyrin repeats		NULL		0	NULL	NULL	NULL	gw60_neurobiolaging_23_5_899_s_14	12392794	Unlike p65, RelB and c-Rel, the p50 and p49 subunits result from proteolytic cleavage of their p105 and p100 precursor molecules, respectively, which include C-terminal I B-like ankyrin repeats that inhibit p50 and p49 activity.	transcription
57130	5	335353	7	NULL	NULL	0	NULL	statement 3			inhibit					p50		activity of			NULL		0	NULL	NULL	NULL	gw60_neurobiolaging_23_5_899_s_14	12392794	Unlike p65, RelB and c-Rel, the p50 and p49 subunits result from proteolytic cleavage of their p105 and p100 precursor molecules, respectively, which include C-terminal I B-like ankyrin repeats that inhibit p50 and p49 activity.	transcription
57131	6	335353	7	NULL	NULL	0	NULL	statement 4			inhibit					p49		activity of			NULL		0	NULL	NULL	NULL	gw60_neurobiolaging_23_5_899_s_14	12392794	Unlike p65, RelB and c-Rel, the p50 and p49 subunits result from proteolytic cleavage of their p105 and p100 precursor molecules, respectively, which include C-terminal I B-like ankyrin repeats that inhibit p50 and p49 activity.	transcription
78237	1	335354	6	NULL	NULL	0	NULL	NF-kappaB	GP		regulate		transcriptionally			beta interferon	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_24_9113_s_145	11094063	It has also been observed that expression of beta interferon, which is transcriptionally regulated by NF-kappaB, is increased in mice with disruptions of the p50 gene ( 19), while in mice with elevated constitutive levels of p50 due to p105 gene disruption, NF-kappaB-regulated cytokine production is increased in some cell types and suppressed in others ( 9).	transcription
78238	2	335354	6	NULL	NULL	NULL	NULL	p50	GP	disruption of	increases					statement 1	process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_24_9113_s_145	11094063	It has also been observed that expression of beta interferon, which is transcriptionally regulated by NF-kappaB, is increased in mice with disruptions of the p50 gene ( 19), while in mice with elevated constitutive levels of p50 due to p105 gene disruption, NF-kappaB-regulated cytokine production is increased in some cell types and suppressed in others ( 9).	transcription
78239	3	335354	6	NULL	NULL	0	NULL	p105	GP	disruption of	increases					p50	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_24_9113_s_145	11094063	It has also been observed that expression of beta interferon, which is transcriptionally regulated by NF-kappaB, is increased in mice with disruptions of the p50 gene ( 19), while in mice with elevated constitutive levels of p50 due to p105 gene disruption, NF-kappaB-regulated cytokine production is increased in some cell types and suppressed in others ( 9).	transcription
78240	4	335354	6	NULL	NULL	0	NULL	NF-kappaB	GP		regulates					cytokine	Chemical	production of 			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_24_9113_s_145	11094063	It has also been observed that expression of beta interferon, which is transcriptionally regulated by NF-kappaB, is increased in mice with disruptions of the p50 gene ( 19), while in mice with elevated constitutive levels of p50 due to p105 gene disruption, NF-kappaB-regulated cytokine production is increased in some cell types and suppressed in others ( 9).	transcription
57132	1	335354	7	NULL	NULL	0	NULL	NF-kappaB			regulates		transcriptionally			beta interferon		expression of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_24_9113_s_145	11094063	It has also been observed that expression of beta interferon, which is transcriptionally regulated by NF-kappaB, is increased in mice with disruptions of the p50 gene ( 19), while in mice with elevated constitutive levels of p50 due to p105 gene disruption, NF-kappaB-regulated cytokine production is increased in some cell types and suppressed in others ( 9).	transcription
57133	2	335354	7	NULL	NULL	0	NULL	p50 gene		disruption of	increase					beta interferon		expression of			NULL	mice	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_24_9113_s_145	11094063	It has also been observed that expression of beta interferon, which is transcriptionally regulated by NF-kappaB, is increased in mice with disruptions of the p50 gene ( 19), while in mice with elevated constitutive levels of p50 due to p105 gene disruption, NF-kappaB-regulated cytokine production is increased in some cell types and suppressed in others ( 9).	transcription
57134	3	335354	7	NULL	NULL	0	NULL	p105 gene		disruption of	elevates					p50		constitutive levels of			NULL	mice	NULL	NULL	NULL	NULL	gw60_molcellbiol_20_24_9113_s_145	11094063	It has also been observed that expression of beta interferon, which is transcriptionally regulated by NF-kappaB, is increased in mice with disruptions of the p50 gene ( 19), while in mice with elevated constitutive levels of p50 due to p105 gene disruption, NF-kappaB-regulated cytokine production is increased in some cell types and suppressed in others ( 9).	transcription
57135	4	335354	7	NULL	NULL	0	NULL	NF-kappaB			regulates					cytokine		production of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_24_9113_s_145	11094063	It has also been observed that expression of beta interferon, which is transcriptionally regulated by NF-kappaB, is increased in mice with disruptions of the p50 gene ( 19), while in mice with elevated constitutive levels of p50 due to p105 gene disruption, NF-kappaB-regulated cytokine production is increased in some cell types and suppressed in others ( 9).	transcription
57136	5	335354	7	NULL	NULL	0	NULL	statement 3			leads to					statement 4					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_24_9113_s_145	11094063	It has also been observed that expression of beta interferon, which is transcriptionally regulated by NF-kappaB, is increased in mice with disruptions of the p50 gene ( 19), while in mice with elevated constitutive levels of p50 due to p105 gene disruption, NF-kappaB-regulated cytokine production is increased in some cell types and suppressed in others ( 9).	transcription
78241	1	335356	6	NULL	NULL	0	NULL	p105	GP		is processed to					p50					NULL	Yeast	0	NULL	NULL	NULL	gw60_jbiolchem_273_3_1409_s_117	9430676	As shown previously, p105 is processed to p50 in yeast (Fig.  1,  lane 1), but a mutation in the beta-type subunit,  pre1-1 ( 59), that decreases the chymotrypsin-like peptide hydrolysis activity of the proteasome blocks the formation of the mature p50 product (Fig.  1,  lane 2; Fig.  6).	transcription
78279	2	335356	6	NULL	NULL	0	NULL	proteasome	CellComponent		hydrolyze					chymotrypsin-like peptide	AminoAcid				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_3_1409_s_117	9430676	As shown previously, p105 is processed to p50 in yeast (Fig.  1,  lane 1), but a mutation in the beta-type subunit,  pre1-1 ( 59), that decreases the chymotrypsin-like peptide hydrolysis activity of the proteasome blocks the formation of the mature p50 product (Fig.  1,  lane 2; Fig.  6).	transcription
78280	3	335356	6	NULL	NULL	0	NULL	pre1-1	GP	mutation of	decreases					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_3_1409_s_117	9430676	As shown previously, p105 is processed to p50 in yeast (Fig.  1,  lane 1), but a mutation in the beta-type subunit,  pre1-1 ( 59), that decreases the chymotrypsin-like peptide hydrolysis activity of the proteasome blocks the formation of the mature p50 product (Fig.  1,  lane 2; Fig.  6).	transcription
78281	4	335356	6	NULL	NULL	0	NULL	statement 2	process		decreases					p50 	GP	formation of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_3_1409_s_117	9430676	As shown previously, p105 is processed to p50 in yeast (Fig.  1,  lane 1), but a mutation in the beta-type subunit,  pre1-1 ( 59), that decreases the chymotrypsin-like peptide hydrolysis activity of the proteasome blocks the formation of the mature p50 product (Fig.  1,  lane 2; Fig.  6).	transcription
57137	1	335356	7	NULL	NULL	0	NULL	 p105			processed to					p50					NULL	yeast	0	NULL	NULL	NULL	gw60_jbiolchem_273_3_1409_s_117	9430676	As shown previously, p105 is processed to p50 in yeast (Fig.  1,  lane 1), but a mutation in the beta-type subunit,  pre1-1 ( 59), that decreases the chymotrypsin-like peptide hydrolysis activity of the proteasome blocks the formation of the mature p50 product (Fig.  1,  lane 2; Fig.  6).	transcription
57138	2	335356	7	NULL	NULL	0	NULL	pre1-1		mutant	decreases			 beta-type subunit		proteasome		chymotrypsin-like peptide hydrolysis activity of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_3_1409_s_117	9430676	As shown previously, p105 is processed to p50 in yeast (Fig.  1,  lane 1), but a mutation in the beta-type subunit,  pre1-1 ( 59), that decreases the chymotrypsin-like peptide hydrolysis activity of the proteasome blocks the formation of the mature p50 product (Fig.  1,  lane 2; Fig.  6).	transcription
57139	3	335356	7	NULL	NULL	0	NULL	statement 2			blocks					p50		formation of mature			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_3_1409_s_117	9430676	As shown previously, p105 is processed to p50 in yeast (Fig.  1,  lane 1), but a mutation in the beta-type subunit,  pre1-1 ( 59), that decreases the chymotrypsin-like peptide hydrolysis activity of the proteasome blocks the formation of the mature p50 product (Fig.  1,  lane 2; Fig.  6).	transcription
78282	1	335357	6	NULL	NULL	0	NULL	BCL-3	GP		mediates					p50 homodimer	GP	formation of 			NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_243	10970863	However, after the primary cotranslational event, the intracellular ratio of p50 and p105 may also be influenced either by cellular factors such as BCL-3, which mediates p50 homodimer formation ( Naumann  et al., 1993;  Watanabe  et al., 1997), or by phosphorylation of p105, which triggers degradation of this protein ( MacKichan  et al., 1996;  Belich  et al., 1999;  Heissmeyer  et al., 1999).	transcription
78283	2	335357	6	NULL	NULL	0	NULL	p105 	GP	phosphorylation of 	triggers					p105	GP	degradation of 			NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_243	10970863	However, after the primary cotranslational event, the intracellular ratio of p50 and p105 may also be influenced either by cellular factors such as BCL-3, which mediates p50 homodimer formation ( Naumann  et al., 1993;  Watanabe  et al., 1997), or by phosphorylation of p105, which triggers degradation of this protein ( MacKichan  et al., 1996;  Belich  et al., 1999;  Heissmeyer  et al., 1999).	transcription
57140	1	335357	7	NULL	NULL	0	NULL	BCL-3			influence		may			p50		intracellular ratio of			NULL		NULL	NULL	NULL	NULL	gw60_embo_19_17_4712_s_243	10970863	However, after the primary cotranslational event, the intracellular ratio of p50 and p105 may also be influenced either by cellular factors such as BCL-3, which mediates p50 homodimer formation ( Naumann  et al., 1993;  Watanabe  et al., 1997), or by phosphorylation of p105, which triggers degradation of this protein ( MacKichan  et al., 1996;  Belich  et al., 1999;  Heissmeyer  et al., 1999).	transcription
57141	2	335357	7	NULL	NULL	0	NULL	BCL-3			influence		may			p105		intracellular ratio of			NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_243	10970863	However, after the primary cotranslational event, the intracellular ratio of p50 and p105 may also be influenced either by cellular factors such as BCL-3, which mediates p50 homodimer formation ( Naumann  et al., 1993;  Watanabe  et al., 1997), or by phosphorylation of p105, which triggers degradation of this protein ( MacKichan  et al., 1996;  Belich  et al., 1999;  Heissmeyer  et al., 1999).	transcription
57142	3	335357	7	NULL	NULL	0	NULL	statement 1			occur simulataneous with					statement 2					NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_243	10970863	However, after the primary cotranslational event, the intracellular ratio of p50 and p105 may also be influenced either by cellular factors such as BCL-3, which mediates p50 homodimer formation ( Naumann  et al., 1993;  Watanabe  et al., 1997), or by phosphorylation of p105, which triggers degradation of this protein ( MacKichan  et al., 1996;  Belich  et al., 1999;  Heissmeyer  et al., 1999).	transcription
57143	4	335357	7	NULL	NULL	0	NULL	statement 3			occur after					primary cotranslational event					NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_243	10970863	However, after the primary cotranslational event, the intracellular ratio of p50 and p105 may also be influenced either by cellular factors such as BCL-3, which mediates p50 homodimer formation ( Naumann  et al., 1993;  Watanabe  et al., 1997), or by phosphorylation of p105, which triggers degradation of this protein ( MacKichan  et al., 1996;  Belich  et al., 1999;  Heissmeyer  et al., 1999).	transcription
57144	5	335357	7	NULL	NULL	0	NULL	BCL-3			mediates					p50 homodimer		formation of			NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_243	10970863	However, after the primary cotranslational event, the intracellular ratio of p50 and p105 may also be influenced either by cellular factors such as BCL-3, which mediates p50 homodimer formation ( Naumann  et al., 1993;  Watanabe  et al., 1997), or by phosphorylation of p105, which triggers degradation of this protein ( MacKichan  et al., 1996;  Belich  et al., 1999;  Heissmeyer  et al., 1999).	transcription
57145	6	335357	7	NULL	NULL	0	NULL	p105		phosphorylation of 	triggers					BCL-3		degradation of			NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_243	10970863	However, after the primary cotranslational event, the intracellular ratio of p50 and p105 may also be influenced either by cellular factors such as BCL-3, which mediates p50 homodimer formation ( Naumann  et al., 1993;  Watanabe  et al., 1997), or by phosphorylation of p105, which triggers degradation of this protein ( MacKichan  et al., 1996;  Belich  et al., 1999;  Heissmeyer  et al., 1999).	transcription
57146	7	335357	7	NULL	NULL	0	NULL	statement 6			influence		may			statement 3					NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_243	10970863	However, after the primary cotranslational event, the intracellular ratio of p50 and p105 may also be influenced either by cellular factors such as BCL-3, which mediates p50 homodimer formation ( Naumann  et al., 1993;  Watanabe  et al., 1997), or by phosphorylation of p105, which triggers degradation of this protein ( MacKichan  et al., 1996;  Belich  et al., 1999;  Heissmeyer  et al., 1999).	transcription
57147	8	335357	7	NULL	NULL	0	NULL	statement 3			is an alternative to					statement 7					NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_243	10970863	However, after the primary cotranslational event, the intracellular ratio of p50 and p105 may also be influenced either by cellular factors such as BCL-3, which mediates p50 homodimer formation ( Naumann  et al., 1993;  Watanabe  et al., 1997), or by phosphorylation of p105, which triggers degradation of this protein ( MacKichan  et al., 1996;  Belich  et al., 1999;  Heissmeyer  et al., 1999).	transcription
57148	9	335357	7	NULL	NULL	0	NULL	BCL-3			is a type of					cellular factor					NULL		0	NULL	NULL	NULL	gw60_embo_19_17_4712_s_243	10970863	However, after the primary cotranslational event, the intracellular ratio of p50 and p105 may also be influenced either by cellular factors such as BCL-3, which mediates p50 homodimer formation ( Naumann  et al., 1993;  Watanabe  et al., 1997), or by phosphorylation of p105, which triggers degradation of this protein ( MacKichan  et al., 1996;  Belich  et al., 1999;  Heissmeyer  et al., 1999).	transcription
78284	1	335358	6	NULL	NULL	0	NULL	p105 	GP		resides in					cytosol	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	transcription
78285	2	335358	6	NULL	NULL	0	NULL	p105	GP		contains								ankyrin motif-rich carboxyl-terminal domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	transcription
78475	3	335358	6	NULL	NULL	0	NULL		AminoAcid		degrades into			IkappaBalpha-related domain		NF-kappaB	GP		p50 DNA binding subunit 		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	transcription
78476	4	335358	6	NULL	NULL	0	NULL	RelA	GP		sequestered into					cytoplasm	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	transcription
78477	5	335358	6	NULL	NULL	0	NULL	p105	GP		sequesters					RelA					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	transcription
78478	6	335358	6	NULL	NULL	0	NULL	IkappaBalpha	GP		sequesters					RelA	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	transcription
57149	1	335358	7	NULL	NULL	0	NULL	p105			resides in		exclusively			cytosolic compartment					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	transcription
57150	2	335358	7	NULL	NULL	0	NULL	statement 1			independent of					cellular activation		status of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	transcription
57151	3	335358	7	NULL	NULL	0	NULL	p105			contains								ankyrin motif-rich carboxyl-terminal domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	transcription
57152	4	335358	7	NULL	NULL	0	NULL	statement 3			inhibit					p105		 nuclear expression of	amino-terminal half		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	transcription
57153	5	335358	7	NULL	NULL	0	NULL	statement 3			inhibit					p105		DNA binding activity of	amino-terminal half		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	transcription
57154	6	335358	7	NULL	NULL	0	NULL	 IkappaBalpha-related domain			constitutively					degraded					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	transcription
57155	7	335358	7	NULL	NULL	0	NULL	statement 6			generate					NF-kappaB			p50 DNA binding subunit of		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	transcription
57156	8	335358	7	NULL	NULL	0	NULL	p105			sequesters		physically			RelA 					NULL	cytoplasmic compartment	0	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	transcription
57157	9	335358	7	NULL	NULL	0	NULL	IkappaBalpha			sequesters		physically			RelA 					NULL	cytoplasmic compartment	0	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	transcription
57158	10	335358	7	NULL	NULL	0	NULL	statement 8			is similar to					statement 9					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	transcription
57159	11	335358	7	NULL	NULL	0	NULL	inducible genes			encode					p105 protein					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	transcription
57160	12	335358	7	NULL	NULL	0	NULL	inducible genes			encode					IkappaBalpha					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	transcription
57161	13	335358	7	NULL	NULL	0	NULL	statement 11			contain							functional	NF-kappaB binding sites		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	transcription
57162	14	335358	7	NULL	NULL	0	NULL	statement 12			contain							functional	NF-kappaB binding sites		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_1_9_s_18	7814425	(i) p105 resides exclusively in the cytosolic compartment  independent of the status of cellular  activation( 8 ,  9 ) ; (ii) p105 contains an ankyrin  motif-rich carboxyl-terminal domain that inhibits the nuclear  expression and DNA binding activity of its amino-terminal  half( 8 ,  9 ,  10 ,  11 ,  12 ) ;  this IkappaBalpha-related domain is constitutively degraded in order to  generate the p50 DNA binding subunit of NF-kappaB( 13 ) ; (iii)  p105, like IkappaBalpha, physically sequesters RelA in the cytoplasmic  compartment ( 14 ) ; and (iv) the inducible genes encoding p105  and IkappaBalpha  both contain functional NF-kappaB binding  sites( 15 ,  16 ,  17 ,  18 ) .	transcription
78479	1	335359	6	NULL	NULL	0	NULL	TSA	Chemical		represses					p105 precursor gene	GP				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1693_3_167_s_172	15363630	Since our data show that TSA represses the gene for the p105 precursor of p50 NF- B and activates the STAT1 gene, it may be that the up-regulation of TNF and its receptor  by TSA may represent additional factors that contribute to the apoptotic cell death  induced by TSA.	transcription
78480	2	335359	6	NULL	NULL	0	NULL	TSA	Chemical		activates					STAT1 gene	GP				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1693_3_167_s_172	15363630	Since our data show that TSA represses the gene for the p105 precursor of p50 NF- B and activates the STAT1 gene, it may be that the up-regulation of TNF and its receptor  by TSA may represent additional factors that contribute to the apoptotic cell death  induced by TSA.	transcription
78481	3	335359	6	NULL	NULL	0	NULL	TNF	GP	upregulation of	contribute to					apoptotic cell death	Process				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1693_3_167_s_172	15363630	Since our data show that TSA represses the gene for the p105 precursor of p50 NF- B and activates the STAT1 gene, it may be that the up-regulation of TNF and its receptor  by TSA may represent additional factors that contribute to the apoptotic cell death  induced by TSA.	transcription
78482	4	335359	6	NULL	NULL	0	NULL	TSA	Chemical		induces					apoptotic cell death	Process				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1693_3_167_s_172	15363630	Since our data show that TSA represses the gene for the p105 precursor of p50 NF- B and activates the STAT1 gene, it may be that the up-regulation of TNF and its receptor  by TSA may represent additional factors that contribute to the apoptotic cell death  induced by TSA.	transcription
57163	1	335359	7	NULL	NULL	0	NULL	p105			precursor of					NF-B			p50		NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1693_3_167_s_172	15363630	Since our data show that TSA represses the gene for the p105 precursor of p50 NF- B and activates the STAT1 gene, it may be that the up-regulation of TNF and its receptor  by TSA may represent additional factors that contribute to the apoptotic cell death  induced by TSA.	transcription
57164	2	335359	7	NULL	NULL	0	NULL	TSA			represses					statement 1					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1693_3_167_s_172	15363630	Since our data show that TSA represses the gene for the p105 precursor of p50 NF- B and activates the STAT1 gene, it may be that the up-regulation of TNF and its receptor  by TSA may represent additional factors that contribute to the apoptotic cell death  induced by TSA.	transcription
57165	3	335359	7	NULL	NULL	0	NULL	TSA			activates					STAT1 gene					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1693_3_167_s_172	15363630	Since our data show that TSA represses the gene for the p105 precursor of p50 NF- B and activates the STAT1 gene, it may be that the up-regulation of TNF and its receptor  by TSA may represent additional factors that contribute to the apoptotic cell death  induced by TSA.	transcription
57166	4	335359	7	NULL	NULL	0	NULL	TSA			up-regulate					TNF					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1693_3_167_s_172	15363630	Since our data show that TSA represses the gene for the p105 precursor of p50 NF- B and activates the STAT1 gene, it may be that the up-regulation of TNF and its receptor  by TSA may represent additional factors that contribute to the apoptotic cell death  induced by TSA.	transcription
57167	5	335359	7	NULL	NULL	0	NULL	TSA			up-regulate					TNF receptor					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1693_3_167_s_172	15363630	Since our data show that TSA represses the gene for the p105 precursor of p50 NF- B and activates the STAT1 gene, it may be that the up-regulation of TNF and its receptor  by TSA may represent additional factors that contribute to the apoptotic cell death  induced by TSA.	transcription
57168	6	335359	7	NULL	NULL	0	NULL	TSA			induce					apoptotic cell death					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1693_3_167_s_172	15363630	Since our data show that TSA represses the gene for the p105 precursor of p50 NF- B and activates the STAT1 gene, it may be that the up-regulation of TNF and its receptor  by TSA may represent additional factors that contribute to the apoptotic cell death  induced by TSA.	transcription
57169	7	335359	7	NULL	NULL	0	NULL	statement 4			contribute to		may			statement 6					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1693_3_167_s_172	15363630	Since our data show that TSA represses the gene for the p105 precursor of p50 NF- B and activates the STAT1 gene, it may be that the up-regulation of TNF and its receptor  by TSA may represent additional factors that contribute to the apoptotic cell death  induced by TSA.	transcription
57170	8	335359	7	NULL	NULL	0	NULL	statement 5			contribute to		may			statement 6					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1693_3_167_s_172	15363630	Since our data show that TSA represses the gene for the p105 precursor of p50 NF- B and activates the STAT1 gene, it may be that the up-regulation of TNF and its receptor  by TSA may represent additional factors that contribute to the apoptotic cell death  induced by TSA.	transcription
78483	1	335360	6	NULL	NULL	0	NULL	NF-B1	GP		play a role in					immune response	Process	regulation of 			NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
78484	2	335360	6	NULL	NULL	NULL	NULL	NF-B1	GP		play a role in					inflammatory response	Process	regulation of 			NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
78485	3	335360	6	NULL	NULL	0	NULL	NF-B1	GP		is					p50/ p105	GP				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
78486	4	335360	6	NULL	NULL	0	NULL	NF-B2	GP		play a role in					inflammatory response	Process	regulation of 			NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
78487	5	335360	6	NULL	NULL	0	NULL	NF-B2	GP		play a role in					immune response	Process	regulation of 			NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
78488	6	335360	6	NULL	NULL	0	NULL	NF-B2	GP		is					p52/p100	GP				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
78489	7	335360	6	NULL	NULL	0	NULL	RelA	GP		play a role in					immune response	Process	regulation of 			NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
78490	8	335360	6	NULL	NULL	0	NULL	RelA	GP		play a role in					inflammatory response	Process	regulation of 			NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
78491	9	335360	6	NULL	NULL	0	NULL	RelA	GP		is					p65	GP				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
78492	10	335360	6	NULL	NULL	0	NULL	c-Rel	GP		play a role in					immune response	Process	regulation of 			NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
78493	11	335360	6	NULL	NULL	0	NULL	c-Rel	GP		play a role in					inflammatory response	Process	regulation of 			NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
78494	12	335360	6	NULL	NULL	0	NULL	RelB	GP		play a role in					immune response	Process	regulation of 			NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
78495	13	335360	6	NULL	NULL	NULL	NULL	RelB	GP		play a role in					inflammatory response	Process	regulation of 			NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
78496	14	335360	6	NULL	NULL	0	NULL	NF-B1	GP		play a role in					cell proliferation	Process				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
78497	15	335360	6	NULL	NULL	0	NULL	NF-B1	GP		play a role in					cell death	Process				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
78498	16	335360	6	NULL	NULL	0	NULL	NF-B2	GP		play a role in					cell death	Process				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
78499	17	335360	6	NULL	NULL	0	NULL	NF-B2	GP		play a role in					cell proliferation	Process				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
78500	18	335360	6	NULL	NULL	0	NULL	RelA	GP		play a role in					cell death	Process				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
78501	19	335360	6	NULL	NULL	0	NULL	RelA	GP		play a role in					cell proliferation	Process				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
78502	20	335360	6	NULL	NULL	0	NULL	c-Rel	GP		play a role in					cell death	Process				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
78503	21	335360	6	NULL	NULL	0	NULL	RelB	GP		play a role in					cell proliferation	Process				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
57171	1	335360	7	NULL	NULL	0	NULL	NF- B transcription factors		mammalian	include					NF- B1					NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
57172	2	335360	7	NULL	NULL	0	NULL	NF- B transcription factors		mammalian	include					NF- B2					NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
57173	3	335360	7	NULL	NULL	0	NULL	NF- B transcription factors		mammalian	include					 RelA					NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
57174	4	335360	7	NULL	NULL	0	NULL	NF- B transcription factors		mammalian	include					c-Rel					NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
57175	5	335360	7	NULL	NULL	0	NULL	NF- B transcription factors		mammalian	include					RelB					NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
57176	6	335360	7	NULL	NULL	0	NULL	NF- B1			play important role in					immune response		regulation of			NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
57177	7	335360	7	NULL	NULL	0	NULL	NF- B2			play important role in					immune response		regulation of			NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
57178	8	335360	7	NULL	NULL	0	NULL	 RelA			play important role in					immune response		regulation of			NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
57179	9	335360	7	NULL	NULL	0	NULL	c-Rel			play important role in					immune response		regulation of			NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
57180	10	335360	7	NULL	NULL	0	NULL	RelB			play important role in					immune response		regulation of			NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
57181	11	335360	7	NULL	NULL	0	NULL	NF- B1			play important role in					inflammatory response		regulation of			NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
57182	12	335360	7	NULL	NULL	0	NULL	NF- B2			play important role in					inflammatory response		regulation of			NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
57183	13	335360	7	NULL	NULL	0	NULL	RelA			play important role in					inflammatory response		regulation of			NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
57184	14	335360	7	NULL	NULL	0	NULL	 c-Rel			play important role in					inflammatory response		regulation of			NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
57185	15	335360	7	NULL	NULL	0	NULL	RelB			play important role in					inflammatory response		regulation of			NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
57186	16	335360	7	NULL	NULL	0	NULL	NF- B1			play important role in					cellular proliferation					NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
57187	17	335360	7	NULL	NULL	0	NULL	NF- B2			play important role in					cellular proliferation					NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
57188	18	335360	7	NULL	NULL	0	NULL	RelA			play important role in					cellular proliferation					NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
57189	19	335360	7	NULL	NULL	0	NULL	c-Rel			play important role in					cellular proliferation					NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
57190	20	335360	7	NULL	NULL	0	NULL	RelB 			play important role in					cellular proliferation					NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
57191	21	335360	7	NULL	NULL	0	NULL	NF- B1			play important role in					cell death					NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
57192	22	335360	7	NULL	NULL	0	NULL	NF- B2			play important role in					cell death					NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
57193	23	335360	7	NULL	NULL	0	NULL	RelA			play important role in					cell death					NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
57194	24	335360	7	NULL	NULL	0	NULL	c-Rel			play important role in					cell death					NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
57195	25	335360	7	NULL	NULL	0	NULL	RelB			play important role in					cell death					NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
57196	26	335360	7	NULL	NULL	0	NULL	NF- B1			consist of					p50/ p105					NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
57197	27	335360	7	NULL	NULL	0	NULL	NF- B2			consist of					p52/p100					NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
57198	28	335360	7	NULL	NULL	0	NULL	RelA			consist of					p65					NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_17_0_149_s_282	10358756	The mammalian NF- B transcription factors, which include NF- B1 (p50/ p105), NF- B2  (p52/p100), RelA (p65), c-Rel, and RelB, play important roles in the regulation of  immune and inflammatory responses, cellular proliferation, and cell death (reviewed  in  109,  110,  111).	transcription
57199	1	335361	7	NULL	NULL	0	NULL	NF-kappaBel family of TFs			include					RELA					NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_10_3154_s_128	15933209	Known NF-kappaB target genes   he NF-kappaBel family of TFs, which includes RELA (p65), NF-kappaB1 (p50, p105), NF-kappaB2 (p52, p100), c-REL and RELB, plays a central role in regulating the immune response ( ).	transcription
57200	2	335361	7	NULL	NULL	0	NULL	 NF-kappaBel family of TFs			include					NF-kappaB1					NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_10_3154_s_128	15933209	Known NF-kappaB target genes   he NF-kappaBel family of TFs, which includes RELA (p65), NF-kappaB1 (p50, p105), NF-kappaB2 (p52, p100), c-REL and RELB, plays a central role in regulating the immune response ( ).	transcription
57201	3	335361	7	NULL	NULL	0	NULL	NF-kappaBel family of TFs			include					NF-kappaB2					NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_10_3154_s_128	15933209	Known NF-kappaB target genes   he NF-kappaBel family of TFs, which includes RELA (p65), NF-kappaB1 (p50, p105), NF-kappaB2 (p52, p100), c-REL and RELB, plays a central role in regulating the immune response ( ).	transcription
57202	4	335361	7	NULL	NULL	0	NULL	NF-kappaBel family of TFs			include					c-REL					NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_10_3154_s_128	15933209	Known NF-kappaB target genes   he NF-kappaBel family of TFs, which includes RELA (p65), NF-kappaB1 (p50, p105), NF-kappaB2 (p52, p100), c-REL and RELB, plays a central role in regulating the immune response ( ).	transcription
57203	5	335361	7	NULL	NULL	0	NULL	NF-kappaBel family of TFs			include					RELB					NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_10_3154_s_128	15933209	Known NF-kappaB target genes   he NF-kappaBel family of TFs, which includes RELA (p65), NF-kappaB1 (p50, p105), NF-kappaB2 (p52, p100), c-REL and RELB, plays a central role in regulating the immune response ( ).	transcription
57204	6	335361	7	NULL	NULL	0	NULL	RELA			plays a central role in					immune response		regulating			NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_10_3154_s_128	15933209	Known NF-kappaB target genes   he NF-kappaBel family of TFs, which includes RELA (p65), NF-kappaB1 (p50, p105), NF-kappaB2 (p52, p100), c-REL and RELB, plays a central role in regulating the immune response ( ).	transcription
57205	7	335361	7	NULL	NULL	0	NULL	NF-kappaB1			plays a central role in					immune response		regulating			NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_10_3154_s_128	15933209	Known NF-kappaB target genes   he NF-kappaBel family of TFs, which includes RELA (p65), NF-kappaB1 (p50, p105), NF-kappaB2 (p52, p100), c-REL and RELB, plays a central role in regulating the immune response ( ).	transcription
57206	8	335361	7	NULL	NULL	0	NULL	NF-kappaB2			plays a central role in					immune response		regulating			NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_10_3154_s_128	15933209	Known NF-kappaB target genes   he NF-kappaBel family of TFs, which includes RELA (p65), NF-kappaB1 (p50, p105), NF-kappaB2 (p52, p100), c-REL and RELB, plays a central role in regulating the immune response ( ).	transcription
57207	9	335361	7	NULL	NULL	0	NULL	c-REL			plays a central role in					immune response		regulating			NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_10_3154_s_128	15933209	Known NF-kappaB target genes   he NF-kappaBel family of TFs, which includes RELA (p65), NF-kappaB1 (p50, p105), NF-kappaB2 (p52, p100), c-REL and RELB, plays a central role in regulating the immune response ( ).	transcription
57208	10	335361	7	NULL	NULL	0	NULL	RELB			plays a central role in					immune response		regulating			NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_10_3154_s_128	15933209	Known NF-kappaB target genes   he NF-kappaBel family of TFs, which includes RELA (p65), NF-kappaB1 (p50, p105), NF-kappaB2 (p52, p100), c-REL and RELB, plays a central role in regulating the immune response ( ).	transcription
57209	11	335361	7	NULL	NULL	0	NULL	RelA 			consist of					p65					NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_10_3154_s_128	15933209	Known NF-kappaB target genes   he NF-kappaBel family of TFs, which includes RELA (p65), NF-kappaB1 (p50, p105), NF-kappaB2 (p52, p100), c-REL and RELB, plays a central role in regulating the immune response ( ).	transcription
57210	12	335361	7	NULL	NULL	0	NULL	NF-kappaB1			consist of					p50					NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_10_3154_s_128	15933209	Known NF-kappaB target genes   he NF-kappaBel family of TFs, which includes RELA (p65), NF-kappaB1 (p50, p105), NF-kappaB2 (p52, p100), c-REL and RELB, plays a central role in regulating the immune response ( ).	transcription
57211	13	335361	7	NULL	NULL	0	NULL	NF-kappaB1			consist of					p105					NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_10_3154_s_128	15933209	Known NF-kappaB target genes   he NF-kappaBel family of TFs, which includes RELA (p65), NF-kappaB1 (p50, p105), NF-kappaB2 (p52, p100), c-REL and RELB, plays a central role in regulating the immune response ( ).	transcription
57212	14	335361	7	NULL	NULL	0	NULL	statement 12			occur simulataneous with					statement 13					NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_10_3154_s_128	15933209	Known NF-kappaB target genes   he NF-kappaBel family of TFs, which includes RELA (p65), NF-kappaB1 (p50, p105), NF-kappaB2 (p52, p100), c-REL and RELB, plays a central role in regulating the immune response ( ).	transcription
57213	15	335361	7	NULL	NULL	0	NULL	NF-kappaB2			consist of					p52					NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_10_3154_s_128	15933209	Known NF-kappaB target genes   he NF-kappaBel family of TFs, which includes RELA (p65), NF-kappaB1 (p50, p105), NF-kappaB2 (p52, p100), c-REL and RELB, plays a central role in regulating the immune response ( ).	transcription
57214	16	335361	7	NULL	NULL	0	NULL	NF-kappaB2			consist of					p100					NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_10_3154_s_128	15933209	Known NF-kappaB target genes   he NF-kappaBel family of TFs, which includes RELA (p65), NF-kappaB1 (p50, p105), NF-kappaB2 (p52, p100), c-REL and RELB, plays a central role in regulating the immune response ( ).	transcription
57215	17	335361	7	NULL	NULL	0	NULL	statement 15			occur simulataneous with					statement 16					NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_10_3154_s_128	15933209	Known NF-kappaB target genes   he NF-kappaBel family of TFs, which includes RELA (p65), NF-kappaB1 (p50, p105), NF-kappaB2 (p52, p100), c-REL and RELB, plays a central role in regulating the immune response ( ).	transcription
78683	1	335364	6	NULL	NULL	0	NULL	TLR	GP		induces					IL-10	GP	expression of			NULL	BMDM	0	NULL	NULL	NULL	gw70_pnas_103_9_3274_s_168	16484370	Finally, the finding that p50  NF-kappaB1 and its precursor, p105 NF-kappaB1, contribute to  TLR-induced IL-10 expression in BMDMs in a direct and indirect  ERK-dependent manner, respectively, highlights the utility of the  model described here to study the joint contribution of the  NF-kappaB and ERK pathways in controlling TLR-mediated gene  expression.	transcription
78684	2	335364	6	NULL	NULL	0	NULL	p50 NF-kappaB1	GP		contribute to					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_103_9_3274_s_168	16484370	Finally, the finding that p50  NF-kappaB1 and its precursor, p105 NF-kappaB1, contribute to  TLR-induced IL-10 expression in BMDMs in a direct and indirect  ERK-dependent manner, respectively, highlights the utility of the  model described here to study the joint contribution of the  NF-kappaB and ERK pathways in controlling TLR-mediated gene  expression.	transcription
78685	3	335364	6	NULL	NULL	0	NULL	p105 NF-kappaB1	GP		contribute to					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_103_9_3274_s_168	16484370	Finally, the finding that p50  NF-kappaB1 and its precursor, p105 NF-kappaB1, contribute to  TLR-induced IL-10 expression in BMDMs in a direct and indirect  ERK-dependent manner, respectively, highlights the utility of the  model described here to study the joint contribution of the  NF-kappaB and ERK pathways in controlling TLR-mediated gene  expression.	transcription
78686	4	335364	6	NULL	NULL	0	NULL	p105 NF-kappaB1	GP		is 					p50 NF-kappaB1 precursor	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_103_9_3274_s_168	16484370	Finally, the finding that p50  NF-kappaB1 and its precursor, p105 NF-kappaB1, contribute to  TLR-induced IL-10 expression in BMDMs in a direct and indirect  ERK-dependent manner, respectively, highlights the utility of the  model described here to study the joint contribution of the  NF-kappaB and ERK pathways in controlling TLR-mediated gene  expression.	transcription
57216	1	335364	7	NULL	NULL	0	NULL	TLR			induce					IL-10		expression of			NULL	BMDMs	NULL	NULL	NULL	NULL	gw70_pnas_103_9_3274_s_168	16484370	Finally, the finding that p50  NF-kappaB1 and its precursor, p105 NF-kappaB1, contribute to  TLR-induced IL-10 expression in BMDMs in a direct and indirect  ERK-dependent manner, respectively, highlights the utility of the  model described here to study the joint contribution of the  NF-kappaB and ERK pathways in controlling TLR-mediated gene  expression.	transcription
57217	2	335364	7	NULL	NULL	0	NULL	p50 NF-kappaB1			contribute to					statement 1					NULL		0	NULL	NULL	NULL	gw70_pnas_103_9_3274_s_168	16484370	Finally, the finding that p50  NF-kappaB1 and its precursor, p105 NF-kappaB1, contribute to  TLR-induced IL-10 expression in BMDMs in a direct and indirect  ERK-dependent manner, respectively, highlights the utility of the  model described here to study the joint contribution of the  NF-kappaB and ERK pathways in controlling TLR-mediated gene  expression.	transcription
57218	3	335364	7	NULL	NULL	0	NULL	statement 2			occur through		directly			ERK-dependent manner					NULL		0	NULL	NULL	NULL	gw70_pnas_103_9_3274_s_168	16484370	Finally, the finding that p50  NF-kappaB1 and its precursor, p105 NF-kappaB1, contribute to  TLR-induced IL-10 expression in BMDMs in a direct and indirect  ERK-dependent manner, respectively, highlights the utility of the  model described here to study the joint contribution of the  NF-kappaB and ERK pathways in controlling TLR-mediated gene  expression.	transcription
57219	4	335364	7	NULL	NULL	0	NULL	p105 NF-kappaB1			contribute to					statement 1					NULL		0	NULL	NULL	NULL	gw70_pnas_103_9_3274_s_168	16484370	Finally, the finding that p50  NF-kappaB1 and its precursor, p105 NF-kappaB1, contribute to  TLR-induced IL-10 expression in BMDMs in a direct and indirect  ERK-dependent manner, respectively, highlights the utility of the  model described here to study the joint contribution of the  NF-kappaB and ERK pathways in controlling TLR-mediated gene  expression.	transcription
57220	5	335364	7	NULL	NULL	0	NULL	statement 4			occur through		indirectly			ERK-dependent manner					NULL		0	NULL	NULL	NULL	gw70_pnas_103_9_3274_s_168	16484370	Finally, the finding that p50  NF-kappaB1 and its precursor, p105 NF-kappaB1, contribute to  TLR-induced IL-10 expression in BMDMs in a direct and indirect  ERK-dependent manner, respectively, highlights the utility of the  model described here to study the joint contribution of the  NF-kappaB and ERK pathways in controlling TLR-mediated gene  expression.	transcription
57221	6	335364	7	NULL	NULL	0	NULL	TLR			mediates					gene expression					NULL		0	NULL	NULL	NULL	gw70_pnas_103_9_3274_s_168	16484370	Finally, the finding that p50  NF-kappaB1 and its precursor, p105 NF-kappaB1, contribute to  TLR-induced IL-10 expression in BMDMs in a direct and indirect  ERK-dependent manner, respectively, highlights the utility of the  model described here to study the joint contribution of the  NF-kappaB and ERK pathways in controlling TLR-mediated gene  expression.	transcription
57222	7	335364	7	NULL	NULL	0	NULL	 NF-kappaB 			controls					statement 6					NULL		0	NULL	NULL	NULL	gw70_pnas_103_9_3274_s_168	16484370	Finally, the finding that p50  NF-kappaB1 and its precursor, p105 NF-kappaB1, contribute to  TLR-induced IL-10 expression in BMDMs in a direct and indirect  ERK-dependent manner, respectively, highlights the utility of the  model described here to study the joint contribution of the  NF-kappaB and ERK pathways in controlling TLR-mediated gene  expression.	transcription
57223	8	335364	7	NULL	NULL	0	NULL	ERK pathways			controls					statement 6					NULL		0	NULL	NULL	NULL	gw70_pnas_103_9_3274_s_168	16484370	Finally, the finding that p50  NF-kappaB1 and its precursor, p105 NF-kappaB1, contribute to  TLR-induced IL-10 expression in BMDMs in a direct and indirect  ERK-dependent manner, respectively, highlights the utility of the  model described here to study the joint contribution of the  NF-kappaB and ERK pathways in controlling TLR-mediated gene  expression.	transcription
57224	9	335364	7	NULL	NULL	0	NULL	p105 NF-kappaB1			is a precursor of					p50 NF-kappaB1					NULL		0	NULL	NULL	NULL	gw70_pnas_103_9_3274_s_168	16484370	Finally, the finding that p50  NF-kappaB1 and its precursor, p105 NF-kappaB1, contribute to  TLR-induced IL-10 expression in BMDMs in a direct and indirect  ERK-dependent manner, respectively, highlights the utility of the  model described here to study the joint contribution of the  NF-kappaB and ERK pathways in controlling TLR-mediated gene  expression.	transcription
78687	1	335365	6	NULL	NULL	0	NULL	NF-kappaB subunit	GP		retained in					cytosol	CellComponent				NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_265	10469655	The precursor molecules p105 and p100 retain NF-kappaB subunits in the cytosol (Rice  et al., 1992  ; Mercurio  et al., 1993  ; Naumann  et al., 1993a  ,b) and are critical for the generation of p50 and p52 homodimers, which are bound specifically by the predominantly nuclear IkappaB homologue Bcl-3.	transcription
78688	2	335365	6	NULL	NULL	0	NULL	p105	GP		participate in					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_265	10469655	The precursor molecules p105 and p100 retain NF-kappaB subunits in the cytosol (Rice  et al., 1992  ; Mercurio  et al., 1993  ; Naumann  et al., 1993a  ,b) and are critical for the generation of p50 and p52 homodimers, which are bound specifically by the predominantly nuclear IkappaB homologue Bcl-3.	transcription
78689	3	335365	6	NULL	NULL	0	NULL	p100	GP		participate in					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_265	10469655	The precursor molecules p105 and p100 retain NF-kappaB subunits in the cytosol (Rice  et al., 1992  ; Mercurio  et al., 1993  ; Naumann  et al., 1993a  ,b) and are critical for the generation of p50 and p52 homodimers, which are bound specifically by the predominantly nuclear IkappaB homologue Bcl-3.	transcription
78690	4	335365	6	NULL	NULL	0	NULL	statement 1	Process		is critical for					p50 homodimer	GP	generation of 			NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_265	10469655	The precursor molecules p105 and p100 retain NF-kappaB subunits in the cytosol (Rice  et al., 1992  ; Mercurio  et al., 1993  ; Naumann  et al., 1993a  ,b) and are critical for the generation of p50 and p52 homodimers, which are bound specifically by the predominantly nuclear IkappaB homologue Bcl-3.	transcription
78691	5	335365	6	NULL	NULL	0	NULL	statement 1	Process		is critical for					p52 homodimer	GP	generation of 			NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_265	10469655	The precursor molecules p105 and p100 retain NF-kappaB subunits in the cytosol (Rice  et al., 1992  ; Mercurio  et al., 1993  ; Naumann  et al., 1993a  ,b) and are critical for the generation of p50 and p52 homodimers, which are bound specifically by the predominantly nuclear IkappaB homologue Bcl-3.	transcription
57225	1	335365	7	NULL	NULL	0	NULL	p105			retain					NF-kappaB subunits					NULL	cytosol	0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_265	10469655	The precursor molecules p105 and p100 retain NF-kappaB subunits in the cytosol (Rice  et al., 1992  ; Mercurio  et al., 1993  ; Naumann  et al., 1993a  ,b) and are critical for the generation of p50 and p52 homodimers, which are bound specifically by the predominantly nuclear IkappaB homologue Bcl-3.	transcription
57226	2	335365	7	NULL	NULL	0	NULL	p100			retain					NF-kappaB subunits					NULL	cytosol	0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_265	10469655	The precursor molecules p105 and p100 retain NF-kappaB subunits in the cytosol (Rice  et al., 1992  ; Mercurio  et al., 1993  ; Naumann  et al., 1993a  ,b) and are critical for the generation of p50 and p52 homodimers, which are bound specifically by the predominantly nuclear IkappaB homologue Bcl-3.	transcription
57227	3	335365	7	NULL	NULL	0	NULL	p105			is critical for					p50 homodimer		generation of			NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_265	10469655	The precursor molecules p105 and p100 retain NF-kappaB subunits in the cytosol (Rice  et al., 1992  ; Mercurio  et al., 1993  ; Naumann  et al., 1993a  ,b) and are critical for the generation of p50 and p52 homodimers, which are bound specifically by the predominantly nuclear IkappaB homologue Bcl-3.	transcription
57228	4	335365	7	NULL	NULL	0	NULL	p100 			is critical for					p50 homodimer		generation of			NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_265	10469655	The precursor molecules p105 and p100 retain NF-kappaB subunits in the cytosol (Rice  et al., 1992  ; Mercurio  et al., 1993  ; Naumann  et al., 1993a  ,b) and are critical for the generation of p50 and p52 homodimers, which are bound specifically by the predominantly nuclear IkappaB homologue Bcl-3.	transcription
57229	5	335365	7	NULL	NULL	0	NULL	p105			is critical for					p52 homodimer		generation of			NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_265	10469655	The precursor molecules p105 and p100 retain NF-kappaB subunits in the cytosol (Rice  et al., 1992  ; Mercurio  et al., 1993  ; Naumann  et al., 1993a  ,b) and are critical for the generation of p50 and p52 homodimers, which are bound specifically by the predominantly nuclear IkappaB homologue Bcl-3.	transcription
57230	6	335365	7	NULL	NULL	0	NULL	p100			is critical for					p52 homodimer		generation of			NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_265	10469655	The precursor molecules p105 and p100 retain NF-kappaB subunits in the cytosol (Rice  et al., 1992  ; Mercurio  et al., 1993  ; Naumann  et al., 1993a  ,b) and are critical for the generation of p50 and p52 homodimers, which are bound specifically by the predominantly nuclear IkappaB homologue Bcl-3.	transcription
57231	7	335365	7	NULL	NULL	0	NULL	p50 homodimer			bind		specifically			Bcl-3					NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_265	10469655	The precursor molecules p105 and p100 retain NF-kappaB subunits in the cytosol (Rice  et al., 1992  ; Mercurio  et al., 1993  ; Naumann  et al., 1993a  ,b) and are critical for the generation of p50 and p52 homodimers, which are bound specifically by the predominantly nuclear IkappaB homologue Bcl-3.	transcription
57232	8	335365	7	NULL	NULL	0	NULL	p52 homodimer			bind		specifically			Bcl-3					NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_265	10469655	The precursor molecules p105 and p100 retain NF-kappaB subunits in the cytosol (Rice  et al., 1992  ; Mercurio  et al., 1993  ; Naumann  et al., 1993a  ,b) and are critical for the generation of p50 and p52 homodimers, which are bound specifically by the predominantly nuclear IkappaB homologue Bcl-3.	transcription
57233	9	335365	7	NULL	NULL	0	NULL	Bcl-3			is a type of					nuclear IkappaB homologue					NULL		NULL	NULL	NULL	NULL	gw60_embo_18_17_4766_s_265	10469655	The precursor molecules p105 and p100 retain NF-kappaB subunits in the cytosol (Rice  et al., 1992  ; Mercurio  et al., 1993  ; Naumann  et al., 1993a  ,b) and are critical for the generation of p50 and p52 homodimers, which are bound specifically by the predominantly nuclear IkappaB homologue Bcl-3.	transcription
57234	10	335365	7	NULL	NULL	0	NULL	p105			is a type of					precursor molecule					NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_265	10469655	The precursor molecules p105 and p100 retain NF-kappaB subunits in the cytosol (Rice  et al., 1992  ; Mercurio  et al., 1993  ; Naumann  et al., 1993a  ,b) and are critical for the generation of p50 and p52 homodimers, which are bound specifically by the predominantly nuclear IkappaB homologue Bcl-3.	transcription
57235	11	335365	7	NULL	NULL	0	NULL	p100			is a type of					precursor molecule					NULL		0	NULL	NULL	NULL	gw60_embo_18_17_4766_s_265	10469655	The precursor molecules p105 and p100 retain NF-kappaB subunits in the cytosol (Rice  et al., 1992  ; Mercurio  et al., 1993  ; Naumann  et al., 1993a  ,b) and are critical for the generation of p50 and p52 homodimers, which are bound specifically by the predominantly nuclear IkappaB homologue Bcl-3.	transcription
78692	1	335366	6	NULL	NULL	0	NULL	1,25-(OH)2-D3	Chemical		reduce					p50	GP	levels of 			NULL	human lymphocytes	0	NULL	NULL	NULL	gw60_febslett_436_3_329_s_128	9801142	Yu et al. have shown that 1,25-(OH)2-D3 can reduce levels of p50 and its precursor p105 in human lymphocytes and they observed reduced binding of PMA-induced nuclear factors to the NF- B binding site of the IL-6 promoter [ 20].	transcription
78693	2	335366	6	NULL	NULL	0	NULL	1,25-(OH)2-D3	Chemical		reduce					p105 precursor gene	GP	levels of 			NULL		0	NULL	NULL	NULL	gw60_febslett_436_3_329_s_128	9801142	Yu et al. have shown that 1,25-(OH)2-D3 can reduce levels of p50 and its precursor p105 in human lymphocytes and they observed reduced binding of PMA-induced nuclear factors to the NF- B binding site of the IL-6 promoter [ 20].	transcription
78694	3	335366	6	NULL	NULL	0	NULL	nuclear factors	GP	PMA-induced	bind					IL-6	GP			NF-B binding site of promoter	NULL		0	NULL	NULL	NULL	gw60_febslett_436_3_329_s_128	9801142	Yu et al. have shown that 1,25-(OH)2-D3 can reduce levels of p50 and its precursor p105 in human lymphocytes and they observed reduced binding of PMA-induced nuclear factors to the NF- B binding site of the IL-6 promoter [ 20].	transcription
57246	1	335366	7	NULL	NULL	0	NULL	1,25-(OH)2-D3			reduce					p50		levels of			NULL	human lymphocytes	NULL	NULL	NULL	NULL	gw60_febslett_436_3_329_s_128	9801142	Yu et al. have shown that 1,25-(OH)2-D3 can reduce levels of p50 and its precursor p105 in human lymphocytes and they observed reduced binding of PMA-induced nuclear factors to the NF- B binding site of the IL-6 promoter [ 20].	transcription
57247	2	335366	7	NULL	NULL	0	NULL	1,25-(OH)2-D3			reduce					precursor p105		levels of			NULL	human lymphocytes	NULL	NULL	NULL	NULL	gw60_febslett_436_3_329_s_128	9801142	Yu et al. have shown that 1,25-(OH)2-D3 can reduce levels of p50 and its precursor p105 in human lymphocytes and they observed reduced binding of PMA-induced nuclear factors to the NF- B binding site of the IL-6 promoter [ 20].	transcription
57248	3	335366	7	NULL	NULL	0	NULL	PMA			induce					nuclear factors					NULL		0	NULL	NULL	NULL	gw60_febslett_436_3_329_s_128	9801142	Yu et al. have shown that 1,25-(OH)2-D3 can reduce levels of p50 and its precursor p105 in human lymphocytes and they observed reduced binding of PMA-induced nuclear factors to the NF- B binding site of the IL-6 promoter [ 20].	transcription
57249	4	335366	7	NULL	NULL	0	NULL	statement 3			bind		reduced			IL-6				NF- B binding site of promoter	NULL		0	NULL	NULL	NULL	gw60_febslett_436_3_329_s_128	9801142	Yu et al. have shown that 1,25-(OH)2-D3 can reduce levels of p50 and its precursor p105 in human lymphocytes and they observed reduced binding of PMA-induced nuclear factors to the NF- B binding site of the IL-6 promoter [ 20].	transcription
57250	1	335367	7	NULL	NULL	0	NULL	v-Abl			induce					cyclin D1		transcription of;;mouse			NULL	293T cells	0	NULL	NULL	NULL	gw60_molcellbiol_22_15_5563_s_233	12101248	The role of NF-kappaB1 in v-Abl-induced cyclin D1 transcription was assessed by cotransfecting 293T cells with mouse  cyclin D1 promoter reporter constructs (Fig.  10A) and expression vectors encoding v-Abl and the p50 or p105 form of NF-kappaB1.	transcription
78695	1	335368	6	NULL	NULL	0	NULL	v-Abl	GP		induces					cyclin D1	GP	transcription of 			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_15_5563_s_237	12101248	In contrast to RelA (lane 9), expression vectors for either the p105 or p50 form of NF-kappaB1 inhibited v-Abl-induced  cyclin D1 transcription (compare lanes 16 and 17 with lane 7), and this repression was mediated predominantly through the kappaB element (compare lanes 20 and 21 with lane 11).	transcription
78696	2	335368	6	NULL	NULL	0	NULL		GP		represses				kappa B element	statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_15_5563_s_237	12101248	In contrast to RelA (lane 9), expression vectors for either the p105 or p50 form of NF-kappaB1 inhibited v-Abl-induced  cyclin D1 transcription (compare lanes 16 and 17 with lane 7), and this repression was mediated predominantly through the kappaB element (compare lanes 20 and 21 with lane 11).	transcription
57251	1	335368	7	NULL	NULL	0	NULL	v-Abl			induce					cyclin D1		transcription of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_15_5563_s_237	12101248	In contrast to RelA (lane 9), expression vectors for either the p105 or p50 form of NF-kappaB1 inhibited v-Abl-induced  cyclin D1 transcription (compare lanes 16 and 17 with lane 7), and this repression was mediated predominantly through the kappaB element (compare lanes 20 and 21 with lane 11).	transcription
57252	2	335368	7	NULL	NULL	0	NULL	NF-kappaB1			inhibits					statement 1					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_15_5563_s_237	12101248	In contrast to RelA (lane 9), expression vectors for either the p105 or p50 form of NF-kappaB1 inhibited v-Abl-induced  cyclin D1 transcription (compare lanes 16 and 17 with lane 7), and this repression was mediated predominantly through the kappaB element (compare lanes 20 and 21 with lane 11).	transcription
57253	3	335368	7	NULL	NULL	0	NULL	statement 2			mediated by		predominantly							kappaB element	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_22_15_5563_s_237	12101248	In contrast to RelA (lane 9), expression vectors for either the p105 or p50 form of NF-kappaB1 inhibited v-Abl-induced  cyclin D1 transcription (compare lanes 16 and 17 with lane 7), and this repression was mediated predominantly through the kappaB element (compare lanes 20 and 21 with lane 11).	transcription
78697	1	335369	6	NULL	NULL	0	NULL	RelB	GP		bind					p100	GP		inhibitory ankyrin containing region		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_2_1405_s_116	11687592	We chose to examine the interaction of RelB with only the inhibitory ankyrin containing regions of p100 and p105, to dissect it from the potential interaction of RelB with the Rel homology domain present in the amino-terminal portions of these atypical inhibitor proteins,  i.e. p52 and p50, respectively.	transcription
78698	2	335369	6	NULL	NULL	0	NULL	RelB	GP		bind					p105	GP		inhibitory ankyrin containing region		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_2_1405_s_116	11687592	We chose to examine the interaction of RelB with only the inhibitory ankyrin containing regions of p100 and p105, to dissect it from the potential interaction of RelB with the Rel homology domain present in the amino-terminal portions of these atypical inhibitor proteins,  i.e. p52 and p50, respectively.	transcription
78699	3	335369	6	NULL	NULL	0	NULL	RelB	GP		bind					p52	GP		Rel homology domain in amino-terminal		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_2_1405_s_116	11687592	We chose to examine the interaction of RelB with only the inhibitory ankyrin containing regions of p100 and p105, to dissect it from the potential interaction of RelB with the Rel homology domain present in the amino-terminal portions of these atypical inhibitor proteins,  i.e. p52 and p50, respectively.	transcription
78700	4	335369	6	NULL	NULL	0	NULL	RelB	GP		bind					p50 	GP		Rel homology domain in amino-terminal		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_2_1405_s_116	11687592	We chose to examine the interaction of RelB with only the inhibitory ankyrin containing regions of p100 and p105, to dissect it from the potential interaction of RelB with the Rel homology domain present in the amino-terminal portions of these atypical inhibitor proteins,  i.e. p52 and p50, respectively.	transcription
57254	1	335369	7	NULL	NULL	0	NULL	RelB			interacts with					p100			inhibitory ankyrin containing regions		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_2_1405_s_116	11687592	We chose to examine the interaction of RelB with only the inhibitory ankyrin containing regions of p100 and p105, to dissect it from the potential interaction of RelB with the Rel homology domain present in the amino-terminal portions of these atypical inhibitor proteins,  i.e. p52 and p50, respectively.	transcription
57255	2	335369	7	NULL	NULL	0	NULL	RelB			interacts with					p105			inhibitory ankyrin containing regions		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_2_1405_s_116	11687592	We chose to examine the interaction of RelB with only the inhibitory ankyrin containing regions of p100 and p105, to dissect it from the potential interaction of RelB with the Rel homology domain present in the amino-terminal portions of these atypical inhibitor proteins,  i.e. p52 and p50, respectively.	transcription
57256	3	335369	7	NULL	NULL	0	NULL	RelB			interacts with					p52			Rel homology domain present in the amino-terminal portions of 		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_2_1405_s_116	11687592	We chose to examine the interaction of RelB with only the inhibitory ankyrin containing regions of p100 and p105, to dissect it from the potential interaction of RelB with the Rel homology domain present in the amino-terminal portions of these atypical inhibitor proteins,  i.e. p52 and p50, respectively.	transcription
57257	4	335369	7	NULL	NULL	0	NULL	RelB			interacts with					p50			Rel homology domain present in the amino-terminal portions of 		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_2_1405_s_116	11687592	We chose to examine the interaction of RelB with only the inhibitory ankyrin containing regions of p100 and p105, to dissect it from the potential interaction of RelB with the Rel homology domain present in the amino-terminal portions of these atypical inhibitor proteins,  i.e. p52 and p50, respectively.	transcription
57258	1	335370	7	NULL	NULL	0	NULL	p105		phosphorylated	bind			tyrosine		phosphatase			active site		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_18_12158_s_189	9115287	Although tyrosine-phosphorylated p105, p62, and p50 most likely bind to the active site of the phosphatase, consistent with the idea of being substrates of DEP-1, we could demonstrate that DEP-1 also engages in protein-protein interactions that require binding determinants other than the catalytic center.	transcription
57259	2	335370	7	NULL	NULL	0	NULL	p62		phosphorylated	bind			tyrosine		phosphatase			active site		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_18_12158_s_189	9115287	Although tyrosine-phosphorylated p105, p62, and p50 most likely bind to the active site of the phosphatase, consistent with the idea of being substrates of DEP-1, we could demonstrate that DEP-1 also engages in protein-protein interactions that require binding determinants other than the catalytic center.	transcription
57260	3	335370	7	NULL	NULL	0	NULL	p50		phosphorylated	bind			tyrosine		phosphatase			active site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_18_12158_s_189	9115287	Although tyrosine-phosphorylated p105, p62, and p50 most likely bind to the active site of the phosphatase, consistent with the idea of being substrates of DEP-1, we could demonstrate that DEP-1 also engages in protein-protein interactions that require binding determinants other than the catalytic center.	transcription
57261	5	335370	7	NULL	NULL	0	NULL	DEP-1			engages in					statement 4					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_18_12158_s_189	9115287	Although tyrosine-phosphorylated p105, p62, and p50 most likely bind to the active site of the phosphatase, consistent with the idea of being substrates of DEP-1, we could demonstrate that DEP-1 also engages in protein-protein interactions that require binding determinants other than the catalytic center.	transcription
57262	4	335370	7	NULL	NULL	0	NULL	protein			interacts with					protein					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_18_12158_s_189	9115287	Although tyrosine-phosphorylated p105, p62, and p50 most likely bind to the active site of the phosphatase, consistent with the idea of being substrates of DEP-1, we could demonstrate that DEP-1 also engages in protein-protein interactions that require binding determinants other than the catalytic center.	transcription
57263	6	335370	7	NULL	NULL	0	NULL	statement 5			require					binding determinants					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_18_12158_s_189	9115287	Although tyrosine-phosphorylated p105, p62, and p50 most likely bind to the active site of the phosphatase, consistent with the idea of being substrates of DEP-1, we could demonstrate that DEP-1 also engages in protein-protein interactions that require binding determinants other than the catalytic center.	transcription
57264	7	335370	7	NULL	NULL	0	NULL	p105		phosphorylated	is a substrate of			tyrosine		DEP-1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_18_12158_s_189	9115287	Although tyrosine-phosphorylated p105, p62, and p50 most likely bind to the active site of the phosphatase, consistent with the idea of being substrates of DEP-1, we could demonstrate that DEP-1 also engages in protein-protein interactions that require binding determinants other than the catalytic center.	transcription
57265	8	335370	7	NULL	NULL	0	NULL	p62		phosphorylated	is a substrate of			tyrosine		DEP-1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_18_12158_s_189	9115287	Although tyrosine-phosphorylated p105, p62, and p50 most likely bind to the active site of the phosphatase, consistent with the idea of being substrates of DEP-1, we could demonstrate that DEP-1 also engages in protein-protein interactions that require binding determinants other than the catalytic center.	transcription
57266	9	335370	7	NULL	NULL	0	NULL	p50		phosphorylated	is a substrate of			tyrosine		DEP-1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_18_12158_s_189	9115287	Although tyrosine-phosphorylated p105, p62, and p50 most likely bind to the active site of the phosphatase, consistent with the idea of being substrates of DEP-1, we could demonstrate that DEP-1 also engages in protein-protein interactions that require binding determinants other than the catalytic center.	transcription
78701	1	335371	6	NULL	NULL	0	NULL	p105	GP	removal of	produces			COOH termini		p50	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_7_5238_s_19	10671572	In mammalian cells, the NF-kappaB family of proteins can be divided into two classes as follows: one class includes p50 and p52, both of which are produced constitutively by the proteasome-mediated removal of the COOH termini of the precursor proteins p105 and p100, respectively ( 22,  25-27).	transcription
78702	2	335371	6	NULL	NULL	0	NULL	p100	GP	removal of	produces			COOH termini		p52	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_7_5238_s_19	10671572	In mammalian cells, the NF-kappaB family of proteins can be divided into two classes as follows: one class includes p50 and p52, both of which are produced constitutively by the proteasome-mediated removal of the COOH termini of the precursor proteins p105 and p100, respectively ( 22,  25-27).	transcription
78703	3	335371	6	NULL	NULL	0	NULL	statement 1	Process		is mediated by					proteasome	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_7_5238_s_19	10671572	In mammalian cells, the NF-kappaB family of proteins can be divided into two classes as follows: one class includes p50 and p52, both of which are produced constitutively by the proteasome-mediated removal of the COOH termini of the precursor proteins p105 and p100, respectively ( 22,  25-27).	transcription
78704	4	335371	6	NULL	NULL	0	NULL	statement 2	Process		is mediated by					proteasome	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_7_5238_s_19	10671572	In mammalian cells, the NF-kappaB family of proteins can be divided into two classes as follows: one class includes p50 and p52, both of which are produced constitutively by the proteasome-mediated removal of the COOH termini of the precursor proteins p105 and p100, respectively ( 22,  25-27).	transcription
78705	5	335371	6	NULL	NULL	0	NULL	p50	GP		belongs to					NF-kappaB family	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_7_5238_s_19	10671572	In mammalian cells, the NF-kappaB family of proteins can be divided into two classes as follows: one class includes p50 and p52, both of which are produced constitutively by the proteasome-mediated removal of the COOH termini of the precursor proteins p105 and p100, respectively ( 22,  25-27).	transcription
78706	6	335371	6	NULL	NULL	0	NULL	p52	GP		belongs to					NF-kappaB family	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_7_5238_s_19	10671572	In mammalian cells, the NF-kappaB family of proteins can be divided into two classes as follows: one class includes p50 and p52, both of which are produced constitutively by the proteasome-mediated removal of the COOH termini of the precursor proteins p105 and p100, respectively ( 22,  25-27).	transcription
57268	1	335371	7	NULL	NULL	0	NULL	NF-kappaB family			include					p50					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_7_5238_s_19	10671572	In mammalian cells, the NF-kappaB family of proteins can be divided into two classes as follows: one class includes p50 and p52, both of which are produced constitutively by the proteasome-mediated removal of the COOH termini of the precursor proteins p105 and p100, respectively ( 22,  25-27).	transcription
57269	2	335371	7	NULL	NULL	0	NULL	NF-kappaB family			include					p52					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_7_5238_s_19	10671572	In mammalian cells, the NF-kappaB family of proteins can be divided into two classes as follows: one class includes p50 and p52, both of which are produced constitutively by the proteasome-mediated removal of the COOH termini of the precursor proteins p105 and p100, respectively ( 22,  25-27).	transcription
57270	3	335371	7	NULL	NULL	0	NULL	proteasome			mediates					p105		removal of	COOH terminus		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_7_5238_s_19	10671572	In mammalian cells, the NF-kappaB family of proteins can be divided into two classes as follows: one class includes p50 and p52, both of which are produced constitutively by the proteasome-mediated removal of the COOH termini of the precursor proteins p105 and p100, respectively ( 22,  25-27).	transcription
57271	4	335371	7	NULL	NULL	0	NULL	proteasome			mediates					p100		removal of	COOH terminus		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_7_5238_s_19	10671572	In mammalian cells, the NF-kappaB family of proteins can be divided into two classes as follows: one class includes p50 and p52, both of which are produced constitutively by the proteasome-mediated removal of the COOH termini of the precursor proteins p105 and p100, respectively ( 22,  25-27).	transcription
57272	5	335371	7	NULL	NULL	0	NULL	p50			produced by		constitutively			statement 3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_7_5238_s_19	10671572	In mammalian cells, the NF-kappaB family of proteins can be divided into two classes as follows: one class includes p50 and p52, both of which are produced constitutively by the proteasome-mediated removal of the COOH termini of the precursor proteins p105 and p100, respectively ( 22,  25-27).	transcription
57273	6	335371	7	NULL	NULL	0	NULL	p52			produced by		constitutively			statement 4					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_7_5238_s_19	10671572	In mammalian cells, the NF-kappaB family of proteins can be divided into two classes as follows: one class includes p50 and p52, both of which are produced constitutively by the proteasome-mediated removal of the COOH termini of the precursor proteins p105 and p100, respectively ( 22,  25-27).	transcription
57274	7	335371	7	NULL	NULL	0	NULL	p105			is a type of					precursor protein					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_7_5238_s_19	10671572	In mammalian cells, the NF-kappaB family of proteins can be divided into two classes as follows: one class includes p50 and p52, both of which are produced constitutively by the proteasome-mediated removal of the COOH termini of the precursor proteins p105 and p100, respectively ( 22,  25-27).	transcription
57275	8	335371	7	NULL	NULL	0	NULL	p100			is a type of					precursor protein					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_7_5238_s_19	10671572	In mammalian cells, the NF-kappaB family of proteins can be divided into two classes as follows: one class includes p50 and p52, both of which are produced constitutively by the proteasome-mediated removal of the COOH termini of the precursor proteins p105 and p100, respectively ( 22,  25-27).	transcription
78707	1	335372	6	NULL	NULL	0	NULL	RelA	GP		belongs to					NF-kappaB family	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_19_13010_s_22	10224051	NF-kappaB consists of five family members including RelA and c-Rel, which contain transcriptional activation domains p100 and p105 precursor proteins, which are cleaved to the active members, p52 and p50, respectively, and RelB (reviewed in Refs.	transcription
78708	2	335372	6	NULL	NULL	0	NULL	c-Rel	GP		belongs to					NF-kappaB family	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_19_13010_s_22	10224051	NF-kappaB consists of five family members including RelA and c-Rel, which contain transcriptional activation domains p100 and p105 precursor proteins, which are cleaved to the active members, p52 and p50, respectively, and RelB (reviewed in Refs.	transcription
78709	3	335372	6	NULL	NULL	0	NULL	p100	GP		is cleaved to					p52	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_19_13010_s_22	10224051	NF-kappaB consists of five family members including RelA and c-Rel, which contain transcriptional activation domains p100 and p105 precursor proteins, which are cleaved to the active members, p52 and p50, respectively, and RelB (reviewed in Refs.	transcription
78710	4	335372	6	NULL	NULL	0	NULL	p105	GP		is cleaved to					p50	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_19_13010_s_22	10224051	NF-kappaB consists of five family members including RelA and c-Rel, which contain transcriptional activation domains p100 and p105 precursor proteins, which are cleaved to the active members, p52 and p50, respectively, and RelB (reviewed in Refs.	transcription
57276	1	335372	7	NULL	NULL	0	NULL	NF-kappaB			consist of					RelA					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_19_13010_s_22	10224051	NF-kappaB consists of five family members including RelA and c-Rel, which contain transcriptional activation domains p100 and p105 precursor proteins, which are cleaved to the active members, p52 and p50, respectively, and RelB (reviewed in Refs.	transcription
57277	2	335372	7	NULL	NULL	0	NULL	NF-kappaB			consist of					c-Rel					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_19_13010_s_22	10224051	NF-kappaB consists of five family members including RelA and c-Rel, which contain transcriptional activation domains p100 and p105 precursor proteins, which are cleaved to the active members, p52 and p50, respectively, and RelB (reviewed in Refs.	transcription
57278	3	335372	7	NULL	NULL	0	NULL	RelA			contain					p100			transcriptional activation domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_19_13010_s_22	10224051	NF-kappaB consists of five family members including RelA and c-Rel, which contain transcriptional activation domains p100 and p105 precursor proteins, which are cleaved to the active members, p52 and p50, respectively, and RelB (reviewed in Refs.	transcription
57279	4	335372	7	NULL	NULL	0	NULL	c-Rel			contain					p105			transcriptional activation domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_19_13010_s_22	10224051	NF-kappaB consists of five family members including RelA and c-Rel, which contain transcriptional activation domains p100 and p105 precursor proteins, which are cleaved to the active members, p52 and p50, respectively, and RelB (reviewed in Refs.	transcription
57280	5	335372	7	NULL	NULL	0	NULL	p100			is cleaved to			transcriptional activation domain		p52					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_19_13010_s_22	10224051	NF-kappaB consists of five family members including RelA and c-Rel, which contain transcriptional activation domains p100 and p105 precursor proteins, which are cleaved to the active members, p52 and p50, respectively, and RelB (reviewed in Refs.	transcription
57281	6	335372	7	NULL	NULL	0	NULL	p105			is cleaved to			transcriptional activation domain		p50					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_19_13010_s_22	10224051	NF-kappaB consists of five family members including RelA and c-Rel, which contain transcriptional activation domains p100 and p105 precursor proteins, which are cleaved to the active members, p52 and p50, respectively, and RelB (reviewed in Refs.	transcription
78711	1	335373	6	NULL	NULL	0	NULL		GP		inhibits			Ankyrin Repeat		p105	GP	processing of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_138	11350967	Ankyrin Repeat-dependent Inhibition of p105 Processing in Vitro Is Probably Mediated by Anchored p50 Subunits, and Inhibition Is Alleviated by the Presence of the C-terminal Signaling Motif--  We surmised that inhibition of processing which is observed with the increasing number of ankyrin repeats (Fig.  2) is caused by the presence of free p50 and other active NF-kappaB subunits in the HeLa cell extract in which the processing reactions are carried out.	transcription
78712	2	335373	6	NULL	NULL	NULL	NULL	p50 subunit	GP	anchored	mediates					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_138	11350967	Ankyrin Repeat-dependent Inhibition of p105 Processing in Vitro Is Probably Mediated by Anchored p50 Subunits, and Inhibition Is Alleviated by the Presence of the C-terminal Signaling Motif--  We surmised that inhibition of processing which is observed with the increasing number of ankyrin repeats (Fig.  2) is caused by the presence of free p50 and other active NF-kappaB subunits in the HeLa cell extract in which the processing reactions are carried out.	transcription
78713	3	335373	6	NULL	NULL	0	NULL	statement 2	Process		is alleviated by							presence of	C-terminal Signaling Motif		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_138	11350967	Ankyrin Repeat-dependent Inhibition of p105 Processing in Vitro Is Probably Mediated by Anchored p50 Subunits, and Inhibition Is Alleviated by the Presence of the C-terminal Signaling Motif--  We surmised that inhibition of processing which is observed with the increasing number of ankyrin repeats (Fig.  2) is caused by the presence of free p50 and other active NF-kappaB subunits in the HeLa cell extract in which the processing reactions are carried out.	transcription
57282	1	335373	7	NULL	NULL	0	NULL	p105		inhibition of;;processing of	depends on								Ankyrin Repeat		NULL	in vitro;;HeLa cell extract	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_138	11350967	Ankyrin Repeat-dependent Inhibition of p105 Processing in Vitro Is Probably Mediated by Anchored p50 Subunits, and Inhibition Is Alleviated by the Presence of the C-terminal Signaling Motif--  We surmised that inhibition of processing which is observed with the increasing number of ankyrin repeats (Fig.  2) is caused by the presence of free p50 and other active NF-kappaB subunits in the HeLa cell extract in which the processing reactions are carried out.	transcription
57283	2	335373	7	NULL	NULL	0	NULL	statement 1			mediated by		probably			p50 subunits		anchored			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_138	11350967	Ankyrin Repeat-dependent Inhibition of p105 Processing in Vitro Is Probably Mediated by Anchored p50 Subunits, and Inhibition Is Alleviated by the Presence of the C-terminal Signaling Motif--  We surmised that inhibition of processing which is observed with the increasing number of ankyrin repeats (Fig.  2) is caused by the presence of free p50 and other active NF-kappaB subunits in the HeLa cell extract in which the processing reactions are carried out.	transcription
57284	3	335373	7	NULL	NULL	0	NULL	p105		inhibition of	is alleviated by							presence of	C-terminal Signaling Motif		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_138	11350967	Ankyrin Repeat-dependent Inhibition of p105 Processing in Vitro Is Probably Mediated by Anchored p50 Subunits, and Inhibition Is Alleviated by the Presence of the C-terminal Signaling Motif--  We surmised that inhibition of processing which is observed with the increasing number of ankyrin repeats (Fig.  2) is caused by the presence of free p50 and other active NF-kappaB subunits in the HeLa cell extract in which the processing reactions are carried out.	transcription
57285	4	335373	7	NULL	NULL	0	NULL	statement 1			caused by					p50		presence of free			NULL	HeLa cell extract	0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_138	11350967	Ankyrin Repeat-dependent Inhibition of p105 Processing in Vitro Is Probably Mediated by Anchored p50 Subunits, and Inhibition Is Alleviated by the Presence of the C-terminal Signaling Motif--  We surmised that inhibition of processing which is observed with the increasing number of ankyrin repeats (Fig.  2) is caused by the presence of free p50 and other active NF-kappaB subunits in the HeLa cell extract in which the processing reactions are carried out.	transcription
57286	5	335373	7	NULL	NULL	0	NULL	statement 1			caused by					NF-kappaB subunits		active			NULL	HeLa cell extract	0	NULL	NULL	NULL	gw60_jbiolchem_276_29_26769_s_138	11350967	Ankyrin Repeat-dependent Inhibition of p105 Processing in Vitro Is Probably Mediated by Anchored p50 Subunits, and Inhibition Is Alleviated by the Presence of the C-terminal Signaling Motif--  We surmised that inhibition of processing which is observed with the increasing number of ankyrin repeats (Fig.  2) is caused by the presence of free p50 and other active NF-kappaB subunits in the HeLa cell extract in which the processing reactions are carried out.	transcription
57287	1	335376	7	NULL	NULL	0	NULL	NF-kappaB1		mammalian	belongs to					class I members					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_477_s_14	9418895	The mammalian members of this family can be grouped into two classes: class I members, which include NF-kappaB1 (p105/p50) and NF-kappaB2 (p100/p52), are transcribed as precursors (p105 and p100) and then proteolytically processed to yield the DNA binding subunits p50 and p52, respectively, and class II members, which include RelA (p65), c-Rel, and RelB, are not proteolytically processed and contain a transcriptional activation domain in their C termini.	transcription
57288	2	335376	7	NULL	NULL	0	NULL	NF-kappaB1		mammalian	consist of					p105/p50					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_477_s_14	9418895	The mammalian members of this family can be grouped into two classes: class I members, which include NF-kappaB1 (p105/p50) and NF-kappaB2 (p100/p52), are transcribed as precursors (p105 and p100) and then proteolytically processed to yield the DNA binding subunits p50 and p52, respectively, and class II members, which include RelA (p65), c-Rel, and RelB, are not proteolytically processed and contain a transcriptional activation domain in their C termini.	transcription
57289	3	335376	7	NULL	NULL	0	NULL	NF-kappaB2		mammalian	belongs to					class I members					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_477_s_14	9418895	The mammalian members of this family can be grouped into two classes: class I members, which include NF-kappaB1 (p105/p50) and NF-kappaB2 (p100/p52), are transcribed as precursors (p105 and p100) and then proteolytically processed to yield the DNA binding subunits p50 and p52, respectively, and class II members, which include RelA (p65), c-Rel, and RelB, are not proteolytically processed and contain a transcriptional activation domain in their C termini.	transcription
57290	4	335376	7	NULL	NULL	0	NULL	NF-kappaB2		mammalian	consist of					p100/p52					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_1_477_s_14	9418895	The mammalian members of this family can be grouped into two classes: class I members, which include NF-kappaB1 (p105/p50) and NF-kappaB2 (p100/p52), are transcribed as precursors (p105 and p100) and then proteolytically processed to yield the DNA binding subunits p50 and p52, respectively, and class II members, which include RelA (p65), c-Rel, and RelB, are not proteolytically processed and contain a transcriptional activation domain in their C termini.	transcription
57291	5	335376	7	NULL	NULL	0	NULL	p105			is a precursor of					NF-kappaB1					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_477_s_14	9418895	The mammalian members of this family can be grouped into two classes: class I members, which include NF-kappaB1 (p105/p50) and NF-kappaB2 (p100/p52), are transcribed as precursors (p105 and p100) and then proteolytically processed to yield the DNA binding subunits p50 and p52, respectively, and class II members, which include RelA (p65), c-Rel, and RelB, are not proteolytically processed and contain a transcriptional activation domain in their C termini.	transcription
57292	6	335376	7	NULL	NULL	0	NULL	p100			is a precursor of					NF-kappaB2					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_477_s_14	9418895	The mammalian members of this family can be grouped into two classes: class I members, which include NF-kappaB1 (p105/p50) and NF-kappaB2 (p100/p52), are transcribed as precursors (p105 and p100) and then proteolytically processed to yield the DNA binding subunits p50 and p52, respectively, and class II members, which include RelA (p65), c-Rel, and RelB, are not proteolytically processed and contain a transcriptional activation domain in their C termini.	transcription
57293	7	335376	7	NULL	NULL	0	NULL	NF-kappaB1			processed to		proteolytically			p50					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_477_s_14	9418895	The mammalian members of this family can be grouped into two classes: class I members, which include NF-kappaB1 (p105/p50) and NF-kappaB2 (p100/p52), are transcribed as precursors (p105 and p100) and then proteolytically processed to yield the DNA binding subunits p50 and p52, respectively, and class II members, which include RelA (p65), c-Rel, and RelB, are not proteolytically processed and contain a transcriptional activation domain in their C termini.	transcription
57294	8	335376	7	NULL	NULL	0	NULL	NF-kappaB2			processed to		proteolytically			p52					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_477_s_14	9418895	The mammalian members of this family can be grouped into two classes: class I members, which include NF-kappaB1 (p105/p50) and NF-kappaB2 (p100/p52), are transcribed as precursors (p105 and p100) and then proteolytically processed to yield the DNA binding subunits p50 and p52, respectively, and class II members, which include RelA (p65), c-Rel, and RelB, are not proteolytically processed and contain a transcriptional activation domain in their C termini.	transcription
57295	9	335376	7	NULL	NULL	0	NULL	p50			bind					DNA					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_477_s_14	9418895	The mammalian members of this family can be grouped into two classes: class I members, which include NF-kappaB1 (p105/p50) and NF-kappaB2 (p100/p52), are transcribed as precursors (p105 and p100) and then proteolytically processed to yield the DNA binding subunits p50 and p52, respectively, and class II members, which include RelA (p65), c-Rel, and RelB, are not proteolytically processed and contain a transcriptional activation domain in their C termini.	transcription
57296	10	335376	7	NULL	NULL	0	NULL	p52			bind					DNA					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_477_s_14	9418895	The mammalian members of this family can be grouped into two classes: class I members, which include NF-kappaB1 (p105/p50) and NF-kappaB2 (p100/p52), are transcribed as precursors (p105 and p100) and then proteolytically processed to yield the DNA binding subunits p50 and p52, respectively, and class II members, which include RelA (p65), c-Rel, and RelB, are not proteolytically processed and contain a transcriptional activation domain in their C termini.	transcription
57297	11	335376	7	NULL	NULL	0	NULL	RelA		mammalian	belongs to					class II members					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_477_s_14	9418895	The mammalian members of this family can be grouped into two classes: class I members, which include NF-kappaB1 (p105/p50) and NF-kappaB2 (p100/p52), are transcribed as precursors (p105 and p100) and then proteolytically processed to yield the DNA binding subunits p50 and p52, respectively, and class II members, which include RelA (p65), c-Rel, and RelB, are not proteolytically processed and contain a transcriptional activation domain in their C termini.	transcription
57298	12	335376	7	NULL	NULL	0	NULL	c-Rel		mammalian	belongs to					class II members					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_477_s_14	9418895	The mammalian members of this family can be grouped into two classes: class I members, which include NF-kappaB1 (p105/p50) and NF-kappaB2 (p100/p52), are transcribed as precursors (p105 and p100) and then proteolytically processed to yield the DNA binding subunits p50 and p52, respectively, and class II members, which include RelA (p65), c-Rel, and RelB, are not proteolytically processed and contain a transcriptional activation domain in their C termini.	transcription
57299	13	335376	7	NULL	NULL	0	NULL	RelB		mammalian	belongs to					class II members					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_477_s_14	9418895	The mammalian members of this family can be grouped into two classes: class I members, which include NF-kappaB1 (p105/p50) and NF-kappaB2 (p100/p52), are transcribed as precursors (p105 and p100) and then proteolytically processed to yield the DNA binding subunits p50 and p52, respectively, and class II members, which include RelA (p65), c-Rel, and RelB, are not proteolytically processed and contain a transcriptional activation domain in their C termini.	transcription
57300	14	335376	7	NULL	NULL	0	NULL	RelA			consist of					p65					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_477_s_14	9418895	The mammalian members of this family can be grouped into two classes: class I members, which include NF-kappaB1 (p105/p50) and NF-kappaB2 (p100/p52), are transcribed as precursors (p105 and p100) and then proteolytically processed to yield the DNA binding subunits p50 and p52, respectively, and class II members, which include RelA (p65), c-Rel, and RelB, are not proteolytically processed and contain a transcriptional activation domain in their C termini.	transcription
57301	15	335376	7	NULL	NULL	0	NULL	RelA			does not undergo					proteolytic processing					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_477_s_14	9418895	The mammalian members of this family can be grouped into two classes: class I members, which include NF-kappaB1 (p105/p50) and NF-kappaB2 (p100/p52), are transcribed as precursors (p105 and p100) and then proteolytically processed to yield the DNA binding subunits p50 and p52, respectively, and class II members, which include RelA (p65), c-Rel, and RelB, are not proteolytically processed and contain a transcriptional activation domain in their C termini.	transcription
57302	16	335376	7	NULL	NULL	0	NULL	c-Rel			does not undergo					proteolytic processing					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_477_s_14	9418895	The mammalian members of this family can be grouped into two classes: class I members, which include NF-kappaB1 (p105/p50) and NF-kappaB2 (p100/p52), are transcribed as precursors (p105 and p100) and then proteolytically processed to yield the DNA binding subunits p50 and p52, respectively, and class II members, which include RelA (p65), c-Rel, and RelB, are not proteolytically processed and contain a transcriptional activation domain in their C termini.	transcription
57303	17	335376	7	NULL	NULL	0	NULL	RelB			does not undergo					proteolytic processing					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_477_s_14	9418895	The mammalian members of this family can be grouped into two classes: class I members, which include NF-kappaB1 (p105/p50) and NF-kappaB2 (p100/p52), are transcribed as precursors (p105 and p100) and then proteolytically processed to yield the DNA binding subunits p50 and p52, respectively, and class II members, which include RelA (p65), c-Rel, and RelB, are not proteolytically processed and contain a transcriptional activation domain in their C termini.	transcription
57304	18	335376	7	NULL	NULL	0	NULL	RelA			contains								transcriptional activation domain in C terminus		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_477_s_14	9418895	The mammalian members of this family can be grouped into two classes: class I members, which include NF-kappaB1 (p105/p50) and NF-kappaB2 (p100/p52), are transcribed as precursors (p105 and p100) and then proteolytically processed to yield the DNA binding subunits p50 and p52, respectively, and class II members, which include RelA (p65), c-Rel, and RelB, are not proteolytically processed and contain a transcriptional activation domain in their C termini.	transcription
57305	19	335376	7	NULL	NULL	0	NULL	c-Rel			contains								transcriptional activation domain in C terminus		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_477_s_14	9418895	The mammalian members of this family can be grouped into two classes: class I members, which include NF-kappaB1 (p105/p50) and NF-kappaB2 (p100/p52), are transcribed as precursors (p105 and p100) and then proteolytically processed to yield the DNA binding subunits p50 and p52, respectively, and class II members, which include RelA (p65), c-Rel, and RelB, are not proteolytically processed and contain a transcriptional activation domain in their C termini.	transcription
57306	20	335376	7	NULL	NULL	0	NULL	RelB			contains								transcriptional activation domain in C terminus		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_1_477_s_14	9418895	The mammalian members of this family can be grouped into two classes: class I members, which include NF-kappaB1 (p105/p50) and NF-kappaB2 (p100/p52), are transcribed as precursors (p105 and p100) and then proteolytically processed to yield the DNA binding subunits p50 and p52, respectively, and class II members, which include RelA (p65), c-Rel, and RelB, are not proteolytically processed and contain a transcriptional activation domain in their C termini.	transcription
78714	1	335377	6	NULL	NULL	0	NULL	v-Abl	GP		induces					cyclin D1	GP	transcription of 			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_15_5563_s_262	12101248	While these findings indicate that NF-kappaB1 downregulates v-Abl-induced  cyclin D1 transcription, an inability to obtain  nfkb1-/- pre-B cells that express only an NF-kappaB1 p50-encoded transgene (Nakamura, unpublished) prevented us from determining if the inhibition of  cyclin D1 transcription induced by v-Abl is mediated through the p50 or p105 form of NF-kappaB1.	transcription
78715	2	335377	6	NULL	NULL	0	NULL	NF-kappaB1	GP		downregulates					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_15_5563_s_262	12101248	While these findings indicate that NF-kappaB1 downregulates v-Abl-induced  cyclin D1 transcription, an inability to obtain  nfkb1-/- pre-B cells that express only an NF-kappaB1 p50-encoded transgene (Nakamura, unpublished) prevented us from determining if the inhibition of  cyclin D1 transcription induced by v-Abl is mediated through the p50 or p105 form of NF-kappaB1.	transcription
57307	1	335377	7	NULL	NULL	0	NULL	v-Abl			induce					cyclin D1		transcription of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_15_5563_s_262	12101248	While these findings indicate that NF-kappaB1 downregulates v-Abl-induced  cyclin D1 transcription, an inability to obtain  nfkb1-/- pre-B cells that express only an NF-kappaB1 p50-encoded transgene (Nakamura, unpublished) prevented us from determining if the inhibition of  cyclin D1 transcription induced by v-Abl is mediated through the p50 or p105 form of NF-kappaB1.	transcription
57308	2	335377	7	NULL	NULL	0	NULL	NF-kappaB1			downregulates					statement 1					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_15_5563_s_262	12101248	While these findings indicate that NF-kappaB1 downregulates v-Abl-induced  cyclin D1 transcription, an inability to obtain  nfkb1-/- pre-B cells that express only an NF-kappaB1 p50-encoded transgene (Nakamura, unpublished) prevented us from determining if the inhibition of  cyclin D1 transcription induced by v-Abl is mediated through the p50 or p105 form of NF-kappaB1.	transcription
78286	1	335378	6	NULL	NULL	NULL	NULL	Uracil phosphoribosyltransferase	GP		catalyzes					uracil	Chemical	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_17_6681_s_181	15090651	Uracil phosphoribosyltransferase catalyzes the phosphorylation of uracil or cytidine (step 1 in  Fig. 2).	transcription
78287	2	335378	6	NULL	NULL	0	NULL	Uracil phosphoribosyltransferase	GP		catalyzes					cytidine	NucleicAcid	phosphorylation of			NULL		0	NULL	NULL	NULL	gw70_pnas_101_17_6681_s_181	15090651	Uracil phosphoribosyltransferase catalyzes the phosphorylation of uracil or cytidine (step 1 in  Fig. 2).	transcription
57309	1	335378	7	NULL	NULL	0	NULL	Uracil phosphoribosyltransferase			catalyzes					uracil		phosphorylation of 			NULL		0	NULL	NULL	NULL	gw70_pnas_101_17_6681_s_181	15090651	Uracil phosphoribosyltransferase catalyzes the phosphorylation of uracil or cytidine (step 1 in  Fig. 2).	transcription
57310	2	335378	7	NULL	NULL	0	NULL	Uracil phosphoribosyltransferase			catalyze					cytidine		phosphorylation of			NULL		0	NULL	NULL	NULL	gw70_pnas_101_17_6681_s_181	15090651	Uracil phosphoribosyltransferase catalyzes the phosphorylation of uracil or cytidine (step 1 in  Fig. 2).	transcription
57311	3	335378	7	NULL	NULL	0	NULL	statement 1			is an alternative to					statement 2					NULL		0	NULL	NULL	NULL	gw70_pnas_101_17_6681_s_181	15090651	Uracil phosphoribosyltransferase catalyzes the phosphorylation of uracil or cytidine (step 1 in  Fig. 2).	transcription
78717	1	335379	6	NULL	NULL	0	NULL	cytidine	Chemical		is deaminated to		site specific			uracil	Chemical				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_8_4426_s_2	9671452	The editing of apolipoprotein B (apo-B) mRNA involves the site-specific deamination of cytidine to uracil.	transcription
78718	2	335379	6	NULL	NULL	0	NULL	apo-B mRNA	NucleicAcid	editing of	involves					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_8_4426_s_2	9671452	The editing of apolipoprotein B (apo-B) mRNA involves the site-specific deamination of cytidine to uracil.	transcription
57312	2	335379	7	NULL	NULL	0	NULL	apo-B mRNA		editing of	involves					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_8_4426_s_2	9671452	The editing of apolipoprotein B (apo-B) mRNA involves the site-specific deamination of cytidine to uracil.	transcription
57313	1	335379	7	NULL	NULL	0	NULL	cytidine			deaminated to		site-specifically			uracil					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_18_8_4426_s_2	9671452	The editing of apolipoprotein B (apo-B) mRNA involves the site-specific deamination of cytidine to uracil.	transcription
57314	3	335379	7	NULL	NULL	0	NULL	apo-B			is					apolipoprotein B					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_8_4426_s_2	9671452	The editing of apolipoprotein B (apo-B) mRNA involves the site-specific deamination of cytidine to uracil.	transcription
57315	1	335380	7	NULL	NULL	0	NULL	uracil plus uridine			repress					pyrG					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_19_5513_s_175	11544212	Addition of pyrimidines to this strain brought about repression of  pyrG, twofold repression by uracil plus uridine, and almost threefold repression by cytidine.	transcription
57316	2	335380	7	NULL	NULL	0	NULL	cytidine			repress					pyrG					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_19_5513_s_175	11544212	Addition of pyrimidines to this strain brought about repression of  pyrG, twofold repression by uracil plus uridine, and almost threefold repression by cytidine.	transcription
57322	1	335381	7	NULL	NULL	0	NULL	cdd		mutation	does not alter					uracil plus uridine		repression by			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_19_5513_s_177	11544212	Repression by uracil plus uridine was not altered by the  cdd mutation, but cytidine became a more effective repressor (seven- to eightfold repression).	transcription
57323	2	335381	7	NULL	NULL	0	NULL	cytidine			became					effective repressor					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_19_5513_s_177	11544212	Repression by uracil plus uridine was not altered by the  cdd mutation, but cytidine became a more effective repressor (seven- to eightfold repression).	transcription
57324	3	335381	7	NULL	NULL	0	NULL	statement 2			because of					cdd		mutation			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_19_5513_s_177	11544212	Repression by uracil plus uridine was not altered by the  cdd mutation, but cytidine became a more effective repressor (seven- to eightfold repression).	transcription
78288	1	335382	6	NULL	NULL	0	NULL	Uracil	NucleicAcid		is removed from					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	abs-batch0560-0569_j-virol_80_2_16378989_s_4	16378989	UNG initiates the removal of uracils from DNA,  and this has been proposed to be important both for reverse transcription  and as a mediator to the antiviral effect of virion-incorporated Apobec3G,  a cytidine deaminase that generates numerous uracils in the viral DNA  during virus replication.	transcription
78719	2	335382	6	NULL	NULL	0	NULL	UNG	Chemical		initiates					statement 1	Process				NULL		0	NULL	NULL	NULL	abs-batch0560-0569_j-virol_80_2_16378989_s_4	16378989	UNG initiates the removal of uracils from DNA,  and this has been proposed to be important both for reverse transcription  and as a mediator to the antiviral effect of virion-incorporated Apobec3G,  a cytidine deaminase that generates numerous uracils in the viral DNA  during virus replication.	transcription
78720	3	335382	6	NULL	NULL	0	NULL	virion-incorporated Apobec3G,	GP		generates					uracil	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0560-0569_j-virol_80_2_16378989_s_4	16378989	UNG initiates the removal of uracils from DNA,  and this has been proposed to be important both for reverse transcription  and as a mediator to the antiviral effect of virion-incorporated Apobec3G,  a cytidine deaminase that generates numerous uracils in the viral DNA  during virus replication.	transcription
78721	4	335382	6	NULL	NULL	0	NULL	statement 3	Process		occurs during					virus	Organism	replication of 			NULL		0	NULL	NULL	NULL	abs-batch0560-0569_j-virol_80_2_16378989_s_4	16378989	UNG initiates the removal of uracils from DNA,  and this has been proposed to be important both for reverse transcription  and as a mediator to the antiviral effect of virion-incorporated Apobec3G,  a cytidine deaminase that generates numerous uracils in the viral DNA  during virus replication.	transcription
78722	5	335382	6	NULL	NULL	0	NULL	virion-incorporated Apobec3G,	GP		is a type of					cytidine deaminase	GP				NULL		0	NULL	NULL	NULL	abs-batch0560-0569_j-virol_80_2_16378989_s_4	16378989	UNG initiates the removal of uracils from DNA,  and this has been proposed to be important both for reverse transcription  and as a mediator to the antiviral effect of virion-incorporated Apobec3G,  a cytidine deaminase that generates numerous uracils in the viral DNA  during virus replication.	transcription
57325	1	335382	7	NULL	NULL	0	NULL	Uracils			removed from					DNA					NULL		0	NULL	NULL	NULL	abs-batch0560-0569_j-virol_80_2_16378989_s_4	16378989	UNG initiates the removal of uracils from DNA,  and this has been proposed to be important both for reverse transcription  and as a mediator to the antiviral effect of virion-incorporated Apobec3G,  a cytidine deaminase that generates numerous uracils in the viral DNA  during virus replication.	transcription
57326	2	335382	7	NULL	NULL	0	NULL	UNG			initiates					statement 1					NULL		0	NULL	NULL	NULL	abs-batch0560-0569_j-virol_80_2_16378989_s_4	16378989	UNG initiates the removal of uracils from DNA,  and this has been proposed to be important both for reverse transcription  and as a mediator to the antiviral effect of virion-incorporated Apobec3G,  a cytidine deaminase that generates numerous uracils in the viral DNA  during virus replication.	transcription
57327	3	335382	7	NULL	NULL	0	NULL	statement 2			is important for					reverse transcription					NULL		0	NULL	NULL	NULL	abs-batch0560-0569_j-virol_80_2_16378989_s_4	16378989	UNG initiates the removal of uracils from DNA,  and this has been proposed to be important both for reverse transcription  and as a mediator to the antiviral effect of virion-incorporated Apobec3G,  a cytidine deaminase that generates numerous uracils in the viral DNA  during virus replication.	transcription
57328	4	335382	7	NULL	NULL	0	NULL	virion			incorporate					Apobec3G					NULL		0	NULL	NULL	NULL	abs-batch0560-0569_j-virol_80_2_16378989_s_4	16378989	UNG initiates the removal of uracils from DNA,  and this has been proposed to be important both for reverse transcription  and as a mediator to the antiviral effect of virion-incorporated Apobec3G,  a cytidine deaminase that generates numerous uracils in the viral DNA  during virus replication.	transcription
57329	5	335382	7	NULL	NULL	0	NULL	statement 2			mediate					statement 4		antiviral effect of 			NULL		NULL	NULL	NULL	NULL	abs-batch0560-0569_j-virol_80_2_16378989_s_4	16378989	UNG initiates the removal of uracils from DNA,  and this has been proposed to be important both for reverse transcription  and as a mediator to the antiviral effect of virion-incorporated Apobec3G,  a cytidine deaminase that generates numerous uracils in the viral DNA  during virus replication.	transcription
57330	6	335382	7	NULL	NULL	0	NULL	Apobec3G			is a type of					 cytidine deaminase					NULL		0	NULL	NULL	NULL	abs-batch0560-0569_j-virol_80_2_16378989_s_4	16378989	UNG initiates the removal of uracils from DNA,  and this has been proposed to be important both for reverse transcription  and as a mediator to the antiviral effect of virion-incorporated Apobec3G,  a cytidine deaminase that generates numerous uracils in the viral DNA  during virus replication.	transcription
57331	7	335382	7	NULL	NULL	0	NULL	Apobec3G			generates					viral DNA		numerous uracils in			NULL		0	NULL	NULL	NULL	abs-batch0560-0569_j-virol_80_2_16378989_s_4	16378989	UNG initiates the removal of uracils from DNA,  and this has been proposed to be important both for reverse transcription  and as a mediator to the antiviral effect of virion-incorporated Apobec3G,  a cytidine deaminase that generates numerous uracils in the viral DNA  during virus replication.	transcription
57332	8	335382	7	NULL	NULL	0	NULL	statement 7			occur during					virus replication					NULL		0	NULL	NULL	NULL	abs-batch0560-0569_j-virol_80_2_16378989_s_4	16378989	UNG initiates the removal of uracils from DNA,  and this has been proposed to be important both for reverse transcription  and as a mediator to the antiviral effect of virion-incorporated Apobec3G,  a cytidine deaminase that generates numerous uracils in the viral DNA  during virus replication.	transcription
78681	1	335383	6	NULL	NULL	0	NULL	AID	GP		is					activation-induced cytidine deaminase	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_103_32_12081_s_18	16873544	The transcription-coupled deamination of cytosines by activation-induced cytidine deaminase (AID) leads to uracil that may be processed to abasic sites or strand breaks by the excision repair pathway, i.e., uracil- N-glycosylase ( ,  ).	transcription
78682	2	335383	6	NULL	NULL	0	NULL	AID	GP		leads to					cytosine	Chemical	deamination of			NULL		0	NULL	NULL	NULL	gw70_pnas_103_32_12081_s_18	16873544	The transcription-coupled deamination of cytosines by activation-induced cytidine deaminase (AID) leads to uracil that may be processed to abasic sites or strand breaks by the excision repair pathway, i.e., uracil- N-glycosylase ( ,  ).	transcription
78723	3	335383	6	NULL	NULL	0	NULL	statement 2	Process		leads to					uracil	Chemical				NULL		0	NULL	NULL	NULL	gw70_pnas_103_32_12081_s_18	16873544	The transcription-coupled deamination of cytosines by activation-induced cytidine deaminase (AID) leads to uracil that may be processed to abasic sites or strand breaks by the excision repair pathway, i.e., uracil- N-glycosylase ( ,  ).	transcription
57333	1	335383	7	NULL	NULL	0	NULL	activation			induce					cytidine deaminase					NULL		0	NULL	NULL	NULL	gw70_pnas_103_32_12081_s_18	16873544	The transcription-coupled deamination of cytosines by activation-induced cytidine deaminase (AID) leads to uracil that may be processed to abasic sites or strand breaks by the excision repair pathway, i.e., uracil- N-glycosylase ( ,  ).	transcription
57334	2	335383	7	NULL	NULL	0	NULL	cytosines		transcription-coupled deamination of	leads to					uracil					NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_32_12081_s_18	16873544	The transcription-coupled deamination of cytosines by activation-induced cytidine deaminase (AID) leads to uracil that may be processed to abasic sites or strand breaks by the excision repair pathway, i.e., uracil- N-glycosylase ( ,  ).	transcription
57335	3	335383	7	NULL	NULL	0	NULL	uracil			be processed to		may							abasic sites	NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_32_12081_s_18	16873544	The transcription-coupled deamination of cytosines by activation-induced cytidine deaminase (AID) leads to uracil that may be processed to abasic sites or strand breaks by the excision repair pathway, i.e., uracil- N-glycosylase ( ,  ).	transcription
57336	4	335383	7	NULL	NULL	0	NULL	uracil			be processed to		may			strand breaks by the excision repair pathway					NULL		0	NULL	NULL	NULL	gw70_pnas_103_32_12081_s_18	16873544	The transcription-coupled deamination of cytosines by activation-induced cytidine deaminase (AID) leads to uracil that may be processed to abasic sites or strand breaks by the excision repair pathway, i.e., uracil- N-glycosylase ( ,  ).	transcription
57338	6	335383	7	NULL	NULL	0	NULL	statement 1			is					AID					NULL		0	NULL	NULL	NULL	gw70_pnas_103_32_12081_s_18	16873544	The transcription-coupled deamination of cytosines by activation-induced cytidine deaminase (AID) leads to uracil that may be processed to abasic sites or strand breaks by the excision repair pathway, i.e., uracil- N-glycosylase ( ,  ).	transcription
57339	5	335383	7	NULL	NULL	0	NULL	statement 2			is carried out by					AID					NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_32_12081_s_18	16873544	The transcription-coupled deamination of cytosines by activation-induced cytidine deaminase (AID) leads to uracil that may be processed to abasic sites or strand breaks by the excision repair pathway, i.e., uracil- N-glycosylase ( ,  ).	transcription
57340	1	335384	7	NULL	NULL	0	NULL	Pol		 polymerase activity of 	mediates					C/G mutations 		generation of			NULL		0	NULL	NULL	NULL	gw70_pnas_102_39_13986_s_35	16172387	We propose that the polymerase activity of Pol  mediates the generation of C/G mutations by replicating over abasic sites formed by uracil-DNA glycosylase-catalyzed excision of the uracil residues generated by activation-induced cytidine deaminase.	transcription
57341	2	335384	7	NULL	NULL	0	NULL	statement 1			occur by							replicating over		abasic sites	NULL		0	NULL	NULL	NULL	gw70_pnas_102_39_13986_s_35	16172387	We propose that the polymerase activity of Pol  mediates the generation of C/G mutations by replicating over abasic sites formed by uracil-DNA glycosylase-catalyzed excision of the uracil residues generated by activation-induced cytidine deaminase.	transcription
57342	3	335384	7	NULL	NULL	0	NULL	uracil-DNA glycosylase			catalyze					uracil residues		excision of			NULL		0	NULL	NULL	NULL	gw70_pnas_102_39_13986_s_35	16172387	We propose that the polymerase activity of Pol  mediates the generation of C/G mutations by replicating over abasic sites formed by uracil-DNA glycosylase-catalyzed excision of the uracil residues generated by activation-induced cytidine deaminase.	transcription
57343	4	335384	7	NULL	NULL	0	NULL				formed by				abasic sites	statement 3					NULL		0	NULL	NULL	NULL	gw70_pnas_102_39_13986_s_35	16172387	We propose that the polymerase activity of Pol  mediates the generation of C/G mutations by replicating over abasic sites formed by uracil-DNA glycosylase-catalyzed excision of the uracil residues generated by activation-induced cytidine deaminase.	transcription
57344	5	335384	7	NULL	NULL	0	NULL	statement 3			generated by					activation-induced cytidine deaminase					NULL		0	NULL	NULL	NULL	gw70_pnas_102_39_13986_s_35	16172387	We propose that the polymerase activity of Pol  mediates the generation of C/G mutations by replicating over abasic sites formed by uracil-DNA glycosylase-catalyzed excision of the uracil residues generated by activation-induced cytidine deaminase.	transcription
78645	1	335385	6	NULL	NULL	0	NULL	Uracil	Chemical		replaces					cytosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_nature_424_6944_99_s_122	12808466	These results are consistent with a model in which the previously demonstrated cytidine  deaminase activity of APOBEC3G leads to the replacement of cytosine by uracil in  the nascent retroviral DNA.	transcription
78646	2	335385	6	NULL	NULL	0	NULL	APOBEC3G	GP		deaminates					cytidine	Chemical				NULL		0	NULL	NULL	NULL	gw70_nature_424_6944_99_s_122	12808466	These results are consistent with a model in which the previously demonstrated cytidine  deaminase activity of APOBEC3G leads to the replacement of cytosine by uracil in  the nascent retroviral DNA.	transcription
78647	3	335385	6	NULL	NULL	0	NULL	statement 2	Process		leads to					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_nature_424_6944_99_s_122	12808466	These results are consistent with a model in which the previously demonstrated cytidine  deaminase activity of APOBEC3G leads to the replacement of cytosine by uracil in  the nascent retroviral DNA.	transcription
57345	1	335385	7	NULL	NULL	0	NULL	APOBEC3G			possess					cytidine deaminase activity					NULL		0	NULL	NULL	NULL	gw70_nature_424_6944_99_s_122	12808466	These results are consistent with a model in which the previously demonstrated cytidine  deaminase activity of APOBEC3G leads to the replacement of cytosine by uracil in  the nascent retroviral DNA.	transcription
57346	3	335385	7	NULL	NULL	0	NULL	statement 1			leads to					statement 3					NULL		NULL	NULL	NULL	NULL	gw70_nature_424_6944_99_s_122	12808466	These results are consistent with a model in which the previously demonstrated cytidine  deaminase activity of APOBEC3G leads to the replacement of cytosine by uracil in  the nascent retroviral DNA.	transcription
57347	2	335385	7	NULL	NULL	0	NULL	cytosine			replaced with					uracil					NULL	nascent retroviral DNA	0	NULL	NULL	NULL	gw70_nature_424_6944_99_s_122	12808466	These results are consistent with a model in which the previously demonstrated cytidine  deaminase activity of APOBEC3G leads to the replacement of cytosine by uracil in  the nascent retroviral DNA.	transcription
78641	1	335386	6	NULL	NULL	0	NULL	cytidine	Chemical		changed to					deoxycytidine	Chemical				NULL		0	NULL	NULL	NULL	gw60_molcell_6_5_1077_s_169	11106747	Modification of cytidine to deoxycytidine (or uracil to thymidine) on either the sense or the antisense strand of the trigger was sufficient to produce a substantial decrease in interference activity (  Figure 5B).	transcription
78642	2	335386	6	NULL	NULL	0	NULL	statement 1	Process		decreases					interference activity	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_6_5_1077_s_169	11106747	Modification of cytidine to deoxycytidine (or uracil to thymidine) on either the sense or the antisense strand of the trigger was sufficient to produce a substantial decrease in interference activity (  Figure 5B).	transcription
78643	3	335386	6	NULL	NULL	0	NULL	Uracil	Chemical		changed to					thymidine	Chemical				NULL		0	NULL	NULL	NULL	gw60_molcell_6_5_1077_s_169	11106747	Modification of cytidine to deoxycytidine (or uracil to thymidine) on either the sense or the antisense strand of the trigger was sufficient to produce a substantial decrease in interference activity (  Figure 5B).	transcription
78644	4	335386	6	NULL	NULL	0	NULL	statement 3	Process		decreases					interference activity	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_6_5_1077_s_169	11106747	Modification of cytidine to deoxycytidine (or uracil to thymidine) on either the sense or the antisense strand of the trigger was sufficient to produce a substantial decrease in interference activity (  Figure 5B).	transcription
57348	1	335386	7	NULL	NULL	0	NULL	cytidine			modified to					deoxycytidine					NULL		0	NULL	NULL	NULL	gw60_molcell_6_5_1077_s_169	11106747	Modification of cytidine to deoxycytidine (or uracil to thymidine) on either the sense or the antisense strand of the trigger was sufficient to produce a substantial decrease in interference activity (  Figure 5B).	transcription
57349	2	335386	7	NULL	NULL	0	NULL	uracil			modified to					thymidine					NULL		0	NULL	NULL	NULL	gw60_molcell_6_5_1077_s_169	11106747	Modification of cytidine to deoxycytidine (or uracil to thymidine) on either the sense or the antisense strand of the trigger was sufficient to produce a substantial decrease in interference activity (  Figure 5B).	transcription
57350	3	335386	7	NULL	NULL	0	NULL	statement 1			produce					interference activity		substantial decrease in			NULL		0	NULL	NULL	NULL	gw60_molcell_6_5_1077_s_169	11106747	Modification of cytidine to deoxycytidine (or uracil to thymidine) on either the sense or the antisense strand of the trigger was sufficient to produce a substantial decrease in interference activity (  Figure 5B).	transcription
57351	4	335386	7	NULL	NULL	0	NULL	statement 2			produce					interference activity		substantial decrease in			NULL		0	NULL	NULL	NULL	gw60_molcell_6_5_1077_s_169	11106747	Modification of cytidine to deoxycytidine (or uracil to thymidine) on either the sense or the antisense strand of the trigger was sufficient to produce a substantial decrease in interference activity (  Figure 5B).	transcription
57352	5	335386	7	NULL	NULL	0	NULL	statement 1			occur in					sense strand					NULL		0	NULL	NULL	NULL	gw60_molcell_6_5_1077_s_169	11106747	Modification of cytidine to deoxycytidine (or uracil to thymidine) on either the sense or the antisense strand of the trigger was sufficient to produce a substantial decrease in interference activity (  Figure 5B).	transcription
57353	6	335386	7	NULL	NULL	0	NULL	statement 1			occur in					antisense strand					NULL		0	NULL	NULL	NULL	gw60_molcell_6_5_1077_s_169	11106747	Modification of cytidine to deoxycytidine (or uracil to thymidine) on either the sense or the antisense strand of the trigger was sufficient to produce a substantial decrease in interference activity (  Figure 5B).	transcription
57354	7	335386	7	NULL	NULL	0	NULL	statement 5			is an alternative to					statement 6					NULL		0	NULL	NULL	NULL	gw60_molcell_6_5_1077_s_169	11106747	Modification of cytidine to deoxycytidine (or uracil to thymidine) on either the sense or the antisense strand of the trigger was sufficient to produce a substantial decrease in interference activity (  Figure 5B).	transcription
57355	8	335386	7	NULL	NULL	0	NULL	statement 2			occur in					sense strand					NULL		0	NULL	NULL	NULL	gw60_molcell_6_5_1077_s_169	11106747	Modification of cytidine to deoxycytidine (or uracil to thymidine) on either the sense or the antisense strand of the trigger was sufficient to produce a substantial decrease in interference activity (  Figure 5B).	transcription
57356	9	335386	7	NULL	NULL	0	NULL	statement 2			occur in					antisense strand					NULL		0	NULL	NULL	NULL	gw60_molcell_6_5_1077_s_169	11106747	Modification of cytidine to deoxycytidine (or uracil to thymidine) on either the sense or the antisense strand of the trigger was sufficient to produce a substantial decrease in interference activity (  Figure 5B).	transcription
57357	10	335386	7	NULL	NULL	0	NULL	statement 8			is an alternative to					statement 9					NULL		0	NULL	NULL	NULL	gw60_molcell_6_5_1077_s_169	11106747	Modification of cytidine to deoxycytidine (or uracil to thymidine) on either the sense or the antisense strand of the trigger was sufficient to produce a substantial decrease in interference activity (  Figure 5B).	transcription
57358	1	335387	7	NULL	NULL	0	NULL	Uracil 			removed in					U-G mismatch					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8765_s_117	15611076	The absence of UDG activity in the cells facilitates subsequent analysis, once it prevents the removal of uracil in U-G mismatch resulting from cytidine deamination, allowing the increase of mutation frequency caused by the activity of deaminase expression.	transcription
57359	2	335387	7	NULL	NULL	0	NULL	statement 1			result from					cytidine deamination					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8765_s_117	15611076	The absence of UDG activity in the cells facilitates subsequent analysis, once it prevents the removal of uracil in U-G mismatch resulting from cytidine deamination, allowing the increase of mutation frequency caused by the activity of deaminase expression.	transcription
57360	3	335387	7	NULL	NULL	0	NULL	UDG activity		absence of	prevents					statement 1					NULL	cells	0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8765_s_117	15611076	The absence of UDG activity in the cells facilitates subsequent analysis, once it prevents the removal of uracil in U-G mismatch resulting from cytidine deamination, allowing the increase of mutation frequency caused by the activity of deaminase expression.	transcription
57361	4	335387	7	NULL	NULL	0	NULL	statement 2			allows					mutation frequency		increase of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8765_s_117	15611076	The absence of UDG activity in the cells facilitates subsequent analysis, once it prevents the removal of uracil in U-G mismatch resulting from cytidine deamination, allowing the increase of mutation frequency caused by the activity of deaminase expression.	transcription
57362	5	335387	7	NULL	NULL	0	NULL	statement 4			caused by					deaminase		activation of;;expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8765_s_117	15611076	The absence of UDG activity in the cells facilitates subsequent analysis, once it prevents the removal of uracil in U-G mismatch resulting from cytidine deamination, allowing the increase of mutation frequency caused by the activity of deaminase expression.	transcription
78635	1	335388	6	NULL	NULL	0	NULL	NTPs	GP		activate					GTP	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_19_19955_s_309	14981084	In previous studies we showed that NTPs activate Gs-proteins in the order of potency GTP > ITP > UTP > XTP > CTP ( ,  ), rendering hypoxanthine, uracil, xanthine, and cytidine nucleotides potential candidates for AC inhibitors.	transcription
78636	2	335388	6	NULL	NULL	0	NULL	NTPs	Chemical		activate					ITP	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_19_19955_s_309	14981084	In previous studies we showed that NTPs activate Gs-proteins in the order of potency GTP > ITP > UTP > XTP > CTP ( ,  ), rendering hypoxanthine, uracil, xanthine, and cytidine nucleotides potential candidates for AC inhibitors.	transcription
78637	3	335388	6	NULL	NULL	0	NULL	NTPs	Chemical		activate					UTP	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_19_19955_s_309	14981084	In previous studies we showed that NTPs activate Gs-proteins in the order of potency GTP > ITP > UTP > XTP > CTP ( ,  ), rendering hypoxanthine, uracil, xanthine, and cytidine nucleotides potential candidates for AC inhibitors.	transcription
78638	4	335388	6	NULL	NULL	0	NULL	NTPs	Chemical		activate					CTP	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_19_19955_s_309	14981084	In previous studies we showed that NTPs activate Gs-proteins in the order of potency GTP > ITP > UTP > XTP > CTP ( ,  ), rendering hypoxanthine, uracil, xanthine, and cytidine nucleotides potential candidates for AC inhibitors.	transcription
57363	1	335388	7	NULL	NULL	0	NULL	NTPs 			activate					Gs-proteins					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_19_19955_s_309	14981084	In previous studies we showed that NTPs activate Gs-proteins in the order of potency GTP > ITP > UTP > XTP > CTP ( ,  ), rendering hypoxanthine, uracil, xanthine, and cytidine nucleotides potential candidates for AC inhibitors.	transcription
57364	2	335388	7	NULL	NULL	0	NULL	hypoxanthine			candidate for		potential			AC inhibitors					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_19_19955_s_309	14981084	In previous studies we showed that NTPs activate Gs-proteins in the order of potency GTP > ITP > UTP > XTP > CTP ( ,  ), rendering hypoxanthine, uracil, xanthine, and cytidine nucleotides potential candidates for AC inhibitors.	transcription
57365	3	335388	7	NULL	NULL	0	NULL	uracil			candidate for		potential			AC inhibitors					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_19_19955_s_309	14981084	In previous studies we showed that NTPs activate Gs-proteins in the order of potency GTP > ITP > UTP > XTP > CTP ( ,  ), rendering hypoxanthine, uracil, xanthine, and cytidine nucleotides potential candidates for AC inhibitors.	transcription
57366	4	335388	7	NULL	NULL	0	NULL	xanthine			candidate for		potential			AC inhibitors					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_19_19955_s_309	14981084	In previous studies we showed that NTPs activate Gs-proteins in the order of potency GTP > ITP > UTP > XTP > CTP ( ,  ), rendering hypoxanthine, uracil, xanthine, and cytidine nucleotides potential candidates for AC inhibitors.	transcription
57367	5	335388	7	NULL	NULL	0	NULL	cytidine nucleotides 			candidate for		potential			AC inhibitors					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_19_19955_s_309	14981084	In previous studies we showed that NTPs activate Gs-proteins in the order of potency GTP > ITP > UTP > XTP > CTP ( ,  ), rendering hypoxanthine, uracil, xanthine, and cytidine nucleotides potential candidates for AC inhibitors.	transcription
57368	1	335389	7	NULL	NULL	0	NULL	ATP			mediate					Cytosine Salvage 					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_9865_s_136	11782482	ATP-mediated Cytosine Salvage-- Strikingly, cytosine was not utilized at all during ATP breakdown (results not shown), showing that the base is not deaminated to uracil and confirming the absence of cytidine phosphorylase and cytosine phosphoribosyltransferase activities in rat brain ( 13).	transcription
57369	2	335389	7	NULL	NULL	0	NULL	cytosine			not utilized during					ATP 		breakdown of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_12_9865_s_136	11782482	ATP-mediated Cytosine Salvage-- Strikingly, cytosine was not utilized at all during ATP breakdown (results not shown), showing that the base is not deaminated to uracil and confirming the absence of cytidine phosphorylase and cytosine phosphoribosyltransferase activities in rat brain ( 13).	transcription
57370	3	335389	7	NULL	NULL	0	NULL	cytosine			is not deaminated to					uracil					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_12_9865_s_136	11782482	ATP-mediated Cytosine Salvage-- Strikingly, cytosine was not utilized at all during ATP breakdown (results not shown), showing that the base is not deaminated to uracil and confirming the absence of cytidine phosphorylase and cytosine phosphoribosyltransferase activities in rat brain ( 13).	transcription
57371	4	335389	7	NULL	NULL	0	NULL	statement 3			confirms					cytidine phosphorylase		absence of			NULL	rat brain	0	NULL	NULL	NULL	gw60_jbiolchem_277_12_9865_s_136	11782482	ATP-mediated Cytosine Salvage-- Strikingly, cytosine was not utilized at all during ATP breakdown (results not shown), showing that the base is not deaminated to uracil and confirming the absence of cytidine phosphorylase and cytosine phosphoribosyltransferase activities in rat brain ( 13).	transcription
57372	5	335389	7	NULL	NULL	0	NULL	statement 3			confirms					cytosine phosphoribosyltransferase		absence of;;activities of			NULL	rat brain	0	NULL	NULL	NULL	gw60_jbiolchem_277_12_9865_s_136	11782482	ATP-mediated Cytosine Salvage-- Strikingly, cytosine was not utilized at all during ATP breakdown (results not shown), showing that the base is not deaminated to uracil and confirming the absence of cytidine phosphorylase and cytosine phosphoribosyltransferase activities in rat brain ( 13).	transcription
78629	1	335390	6	NULL	NULL	0	NULL	APOBEC-1	GP		forms a complex with					ACF	GP				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_20_0_165_s_431	11861601	APOBEC-1 forms a complex with an RNA-binding protein ACF and converts the specific  cytosine at position 6666 of apolipoprotein B mRNA to uracil by its intrinsic cytidine  deaminase activity, giving rise to mRNA encoding the chylomicron component ( 250,  251).	transcription
78630	2	335390	6	NULL	NULL	NULL	NULL	ACF	GP		is a type of					RNA-binding protein	GP				NULL		NULL	NULL	NULL	NULL	gw70_annurevimmunol_20_0_165_s_431	11861601	APOBEC-1 forms a complex with an RNA-binding protein ACF and converts the specific  cytosine at position 6666 of apolipoprotein B mRNA to uracil by its intrinsic cytidine  deaminase activity, giving rise to mRNA encoding the chylomicron component ( 250,  251).	transcription
78631	3	335390	6	NULL	NULL	0	NULL	apolipoprotein B mRNA	NucleicAcid		is converted to					uracil	Chemical				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_20_0_165_s_431	11861601	APOBEC-1 forms a complex with an RNA-binding protein ACF and converts the specific  cytosine at position 6666 of apolipoprotein B mRNA to uracil by its intrinsic cytidine  deaminase activity, giving rise to mRNA encoding the chylomicron component ( 250,  251).	transcription
78632	4	335390	6	NULL	NULL	0	NULL	APOBEC-1	GP		performs					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_20_0_165_s_431	11861601	APOBEC-1 forms a complex with an RNA-binding protein ACF and converts the specific  cytosine at position 6666 of apolipoprotein B mRNA to uracil by its intrinsic cytidine  deaminase activity, giving rise to mRNA encoding the chylomicron component ( 250,  251).	transcription
78633	5	335390	6	NULL	NULL	0	NULL	APOBEC-1	GP		deaminates					cytidine	Chemical				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_20_0_165_s_431	11861601	APOBEC-1 forms a complex with an RNA-binding protein ACF and converts the specific  cytosine at position 6666 of apolipoprotein B mRNA to uracil by its intrinsic cytidine  deaminase activity, giving rise to mRNA encoding the chylomicron component ( 250,  251).	transcription
78634	6	335390	6	NULL	NULL	0	NULL	mRNA	NucleicAcid		encodes					chylomicron component	CellComponent				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_20_0_165_s_431	11861601	APOBEC-1 forms a complex with an RNA-binding protein ACF and converts the specific  cytosine at position 6666 of apolipoprotein B mRNA to uracil by its intrinsic cytidine  deaminase activity, giving rise to mRNA encoding the chylomicron component ( 250,  251).	transcription
57373	1	335390	7	NULL	NULL	0	NULL	APOBEC-1			forms a complex with					ACF					NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_20_0_165_s_431	11861601	APOBEC-1 forms a complex with an RNA-binding protein ACF and converts the specific  cytosine at position 6666 of apolipoprotein B mRNA to uracil by its intrinsic cytidine  deaminase activity, giving rise to mRNA encoding the chylomicron component ( 250,  251).	transcription
57374	2	335390	7	NULL	NULL	0	NULL	ACF			is a type of					RNA-binding protein					NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_20_0_165_s_431	11861601	APOBEC-1 forms a complex with an RNA-binding protein ACF and converts the specific  cytosine at position 6666 of apolipoprotein B mRNA to uracil by its intrinsic cytidine  deaminase activity, giving rise to mRNA encoding the chylomicron component ( 250,  251).	transcription
57375	3	335390	7	NULL	NULL	0	NULL	apolipoprotein B mRNA			converted to				cytosine at position 6666	uracil					NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_20_0_165_s_431	11861601	APOBEC-1 forms a complex with an RNA-binding protein ACF and converts the specific  cytosine at position 6666 of apolipoprotein B mRNA to uracil by its intrinsic cytidine  deaminase activity, giving rise to mRNA encoding the chylomicron component ( 250,  251).	transcription
57376	4	335390	7	NULL	NULL	0	NULL	statement 1			leads to					statement 3					NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_20_0_165_s_431	11861601	APOBEC-1 forms a complex with an RNA-binding protein ACF and converts the specific  cytosine at position 6666 of apolipoprotein B mRNA to uracil by its intrinsic cytidine  deaminase activity, giving rise to mRNA encoding the chylomicron component ( 250,  251).	transcription
57377	5	335390	7	NULL	NULL	0	NULL	statement 3			occur by					cytidine deaminase 		intrinsic activity of			NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_20_0_165_s_431	11861601	APOBEC-1 forms a complex with an RNA-binding protein ACF and converts the specific  cytosine at position 6666 of apolipoprotein B mRNA to uracil by its intrinsic cytidine  deaminase activity, giving rise to mRNA encoding the chylomicron component ( 250,  251).	transcription
57378	6	335390	7	NULL	NULL	0	NULL	statement 5			generates					mRNA					NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_20_0_165_s_431	11861601	APOBEC-1 forms a complex with an RNA-binding protein ACF and converts the specific  cytosine at position 6666 of apolipoprotein B mRNA to uracil by its intrinsic cytidine  deaminase activity, giving rise to mRNA encoding the chylomicron component ( 250,  251).	transcription
57379	7	335390	7	NULL	NULL	0	NULL	mRNA			encodes					chylomicron component					NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_20_0_165_s_431	11861601	APOBEC-1 forms a complex with an RNA-binding protein ACF and converts the specific  cytosine at position 6666 of apolipoprotein B mRNA to uracil by its intrinsic cytidine  deaminase activity, giving rise to mRNA encoding the chylomicron component ( 250,  251).	transcription
57380	1	335391	7	NULL	NULL	0	NULL	adenosine			inhibits		marginally			[3]D-inosine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20935_s_142	10783393	By contrast a 100-fold excess of the naturally occurring nucleosides, adenosine (<1%), xanthosine (35%), uridine (33%), cytidine (<1%), and thymidine (14%), as well as the nucleobases, adenine (6%), hypoxanthine (24%), guanine (26%), xanthine (12%), thymine (<1%), and uracil (1%), only inhibited 1 muM [3]D-inosine marginally (Fig.  7).	transcription
57381	2	335391	7	NULL	NULL	0	NULL	xanthosine			inhibits		marginally			[3]D-inosine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20935_s_142	10783393	By contrast a 100-fold excess of the naturally occurring nucleosides, adenosine (<1%), xanthosine (35%), uridine (33%), cytidine (<1%), and thymidine (14%), as well as the nucleobases, adenine (6%), hypoxanthine (24%), guanine (26%), xanthine (12%), thymine (<1%), and uracil (1%), only inhibited 1 muM [3]D-inosine marginally (Fig.  7).	transcription
57382	3	335391	7	NULL	NULL	0	NULL	uridine			inhibits		marginally			[3]D-inosine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20935_s_142	10783393	By contrast a 100-fold excess of the naturally occurring nucleosides, adenosine (<1%), xanthosine (35%), uridine (33%), cytidine (<1%), and thymidine (14%), as well as the nucleobases, adenine (6%), hypoxanthine (24%), guanine (26%), xanthine (12%), thymine (<1%), and uracil (1%), only inhibited 1 muM [3]D-inosine marginally (Fig.  7).	transcription
57383	4	335391	7	NULL	NULL	0	NULL	cytidine			inhibits		marginally			[3]D-inosine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20935_s_142	10783393	By contrast a 100-fold excess of the naturally occurring nucleosides, adenosine (<1%), xanthosine (35%), uridine (33%), cytidine (<1%), and thymidine (14%), as well as the nucleobases, adenine (6%), hypoxanthine (24%), guanine (26%), xanthine (12%), thymine (<1%), and uracil (1%), only inhibited 1 muM [3]D-inosine marginally (Fig.  7).	transcription
57384	5	335391	7	NULL	NULL	0	NULL	thymidine			inhibits		marginally			[3]D-inosine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20935_s_142	10783393	By contrast a 100-fold excess of the naturally occurring nucleosides, adenosine (<1%), xanthosine (35%), uridine (33%), cytidine (<1%), and thymidine (14%), as well as the nucleobases, adenine (6%), hypoxanthine (24%), guanine (26%), xanthine (12%), thymine (<1%), and uracil (1%), only inhibited 1 muM [3]D-inosine marginally (Fig.  7).	transcription
57385	6	335391	7	NULL	NULL	0	NULL	adenine			inhibits		marginally			[3]D-inosine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20935_s_142	10783393	By contrast a 100-fold excess of the naturally occurring nucleosides, adenosine (<1%), xanthosine (35%), uridine (33%), cytidine (<1%), and thymidine (14%), as well as the nucleobases, adenine (6%), hypoxanthine (24%), guanine (26%), xanthine (12%), thymine (<1%), and uracil (1%), only inhibited 1 muM [3]D-inosine marginally (Fig.  7).	transcription
57386	7	335391	7	NULL	NULL	0	NULL	hypoxanthine			inhibits		marginally			[3]D-inosine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20935_s_142	10783393	By contrast a 100-fold excess of the naturally occurring nucleosides, adenosine (<1%), xanthosine (35%), uridine (33%), cytidine (<1%), and thymidine (14%), as well as the nucleobases, adenine (6%), hypoxanthine (24%), guanine (26%), xanthine (12%), thymine (<1%), and uracil (1%), only inhibited 1 muM [3]D-inosine marginally (Fig.  7).	transcription
57387	8	335391	7	NULL	NULL	0	NULL	guanine			inhibits		marginally			[3]D-inosine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20935_s_142	10783393	By contrast a 100-fold excess of the naturally occurring nucleosides, adenosine (<1%), xanthosine (35%), uridine (33%), cytidine (<1%), and thymidine (14%), as well as the nucleobases, adenine (6%), hypoxanthine (24%), guanine (26%), xanthine (12%), thymine (<1%), and uracil (1%), only inhibited 1 muM [3]D-inosine marginally (Fig.  7).	transcription
57388	9	335391	7	NULL	NULL	0	NULL	xanthine			inhibits		marginally			[3]D-inosine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20935_s_142	10783393	By contrast a 100-fold excess of the naturally occurring nucleosides, adenosine (<1%), xanthosine (35%), uridine (33%), cytidine (<1%), and thymidine (14%), as well as the nucleobases, adenine (6%), hypoxanthine (24%), guanine (26%), xanthine (12%), thymine (<1%), and uracil (1%), only inhibited 1 muM [3]D-inosine marginally (Fig.  7).	transcription
57389	10	335391	7	NULL	NULL	0	NULL	thymine			inhibits		marginally			[3]D-inosine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20935_s_142	10783393	By contrast a 100-fold excess of the naturally occurring nucleosides, adenosine (<1%), xanthosine (35%), uridine (33%), cytidine (<1%), and thymidine (14%), as well as the nucleobases, adenine (6%), hypoxanthine (24%), guanine (26%), xanthine (12%), thymine (<1%), and uracil (1%), only inhibited 1 muM [3]D-inosine marginally (Fig.  7).	transcription
57390	11	335391	7	NULL	NULL	0	NULL	uracil 			inhibits		marginally			[3]D-inosine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20935_s_142	10783393	By contrast a 100-fold excess of the naturally occurring nucleosides, adenosine (<1%), xanthosine (35%), uridine (33%), cytidine (<1%), and thymidine (14%), as well as the nucleobases, adenine (6%), hypoxanthine (24%), guanine (26%), xanthine (12%), thymine (<1%), and uracil (1%), only inhibited 1 muM [3]D-inosine marginally (Fig.  7).	transcription
57391	12	335391	7	NULL	NULL	0	NULL	adenosine			is a type of					naturally occuring nucleoside					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20935_s_142	10783393	By contrast a 100-fold excess of the naturally occurring nucleosides, adenosine (<1%), xanthosine (35%), uridine (33%), cytidine (<1%), and thymidine (14%), as well as the nucleobases, adenine (6%), hypoxanthine (24%), guanine (26%), xanthine (12%), thymine (<1%), and uracil (1%), only inhibited 1 muM [3]D-inosine marginally (Fig.  7).	transcription
57392	13	335391	7	NULL	NULL	0	NULL	xanthosine			is a type of					naturally occuring nucleoside					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20935_s_142	10783393	By contrast a 100-fold excess of the naturally occurring nucleosides, adenosine (<1%), xanthosine (35%), uridine (33%), cytidine (<1%), and thymidine (14%), as well as the nucleobases, adenine (6%), hypoxanthine (24%), guanine (26%), xanthine (12%), thymine (<1%), and uracil (1%), only inhibited 1 muM [3]D-inosine marginally (Fig.  7).	transcription
57393	14	335391	7	NULL	NULL	0	NULL	uridine			is a type of					naturally occuring nucleoside					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20935_s_142	10783393	By contrast a 100-fold excess of the naturally occurring nucleosides, adenosine (<1%), xanthosine (35%), uridine (33%), cytidine (<1%), and thymidine (14%), as well as the nucleobases, adenine (6%), hypoxanthine (24%), guanine (26%), xanthine (12%), thymine (<1%), and uracil (1%), only inhibited 1 muM [3]D-inosine marginally (Fig.  7).	transcription
57394	15	335391	7	NULL	NULL	0	NULL	cytidine			is a type of					naturally occuring nucleoside					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20935_s_142	10783393	By contrast a 100-fold excess of the naturally occurring nucleosides, adenosine (<1%), xanthosine (35%), uridine (33%), cytidine (<1%), and thymidine (14%), as well as the nucleobases, adenine (6%), hypoxanthine (24%), guanine (26%), xanthine (12%), thymine (<1%), and uracil (1%), only inhibited 1 muM [3]D-inosine marginally (Fig.  7).	transcription
57395	16	335391	7	NULL	NULL	0	NULL	thymidine			is a type of					naturally occuring nucleoside					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20935_s_142	10783393	By contrast a 100-fold excess of the naturally occurring nucleosides, adenosine (<1%), xanthosine (35%), uridine (33%), cytidine (<1%), and thymidine (14%), as well as the nucleobases, adenine (6%), hypoxanthine (24%), guanine (26%), xanthine (12%), thymine (<1%), and uracil (1%), only inhibited 1 muM [3]D-inosine marginally (Fig.  7).	transcription
57396	17	335391	7	NULL	NULL	0	NULL	adenine			is a type of					nucleobase					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20935_s_142	10783393	By contrast a 100-fold excess of the naturally occurring nucleosides, adenosine (<1%), xanthosine (35%), uridine (33%), cytidine (<1%), and thymidine (14%), as well as the nucleobases, adenine (6%), hypoxanthine (24%), guanine (26%), xanthine (12%), thymine (<1%), and uracil (1%), only inhibited 1 muM [3]D-inosine marginally (Fig.  7).	transcription
57397	18	335391	7	NULL	NULL	0	NULL	hypoxanthine			is a type of					nucleobase					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20935_s_142	10783393	By contrast a 100-fold excess of the naturally occurring nucleosides, adenosine (<1%), xanthosine (35%), uridine (33%), cytidine (<1%), and thymidine (14%), as well as the nucleobases, adenine (6%), hypoxanthine (24%), guanine (26%), xanthine (12%), thymine (<1%), and uracil (1%), only inhibited 1 muM [3]D-inosine marginally (Fig.  7).	transcription
57398	19	335391	7	NULL	NULL	0	NULL	guanine			is a type of					nucleobase					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20935_s_142	10783393	By contrast a 100-fold excess of the naturally occurring nucleosides, adenosine (<1%), xanthosine (35%), uridine (33%), cytidine (<1%), and thymidine (14%), as well as the nucleobases, adenine (6%), hypoxanthine (24%), guanine (26%), xanthine (12%), thymine (<1%), and uracil (1%), only inhibited 1 muM [3]D-inosine marginally (Fig.  7).	transcription
57399	20	335391	7	NULL	NULL	0	NULL	xanthine			is a type of					nucleobase					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20935_s_142	10783393	By contrast a 100-fold excess of the naturally occurring nucleosides, adenosine (<1%), xanthosine (35%), uridine (33%), cytidine (<1%), and thymidine (14%), as well as the nucleobases, adenine (6%), hypoxanthine (24%), guanine (26%), xanthine (12%), thymine (<1%), and uracil (1%), only inhibited 1 muM [3]D-inosine marginally (Fig.  7).	transcription
57400	21	335391	7	NULL	NULL	0	NULL	thymine			is a type of					nucleobase					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20935_s_142	10783393	By contrast a 100-fold excess of the naturally occurring nucleosides, adenosine (<1%), xanthosine (35%), uridine (33%), cytidine (<1%), and thymidine (14%), as well as the nucleobases, adenine (6%), hypoxanthine (24%), guanine (26%), xanthine (12%), thymine (<1%), and uracil (1%), only inhibited 1 muM [3]D-inosine marginally (Fig.  7).	transcription
57401	22	335391	7	NULL	NULL	0	NULL	uracil			is a type of					nucleobase					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20935_s_142	10783393	By contrast a 100-fold excess of the naturally occurring nucleosides, adenosine (<1%), xanthosine (35%), uridine (33%), cytidine (<1%), and thymidine (14%), as well as the nucleobases, adenine (6%), hypoxanthine (24%), guanine (26%), xanthine (12%), thymine (<1%), and uracil (1%), only inhibited 1 muM [3]D-inosine marginally (Fig.  7).	transcription
78626	1	335392	6	NULL	NULL	0	NULL	RNase-4	GP		prefers					Uracil	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_21_14902_s_116	10329690	Uracil was selected as the base because RNase-4, one of the targets for the inhibitors under development (see below), strongly prefers this pyrimidine over cytosine ( 17), and most of the other mammalian RNases bind uridine and cytidine nucleotides with similar affinity ( 1,  23,  27).	transcription
78627	2	335392	6	NULL	NULL	0	NULL	Uracil	Chemical		is a type of					pyrimidine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_21_14902_s_116	10329690	Uracil was selected as the base because RNase-4, one of the targets for the inhibitors under development (see below), strongly prefers this pyrimidine over cytosine ( 17), and most of the other mammalian RNases bind uridine and cytidine nucleotides with similar affinity ( 1,  23,  27).	transcription
57402	1	335392	7	NULL	NULL	0	NULL	RNases		mammalian	bind					uridine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_21_14902_s_116	10329690	Uracil was selected as the base because RNase-4, one of the targets for the inhibitors under development (see below), strongly prefers this pyrimidine over cytosine ( 17), and most of the other mammalian RNases bind uridine and cytidine nucleotides with similar affinity ( 1,  23,  27).	transcription
57403	2	335392	7	NULL	NULL	0	NULL	RNases		mammalian	bind					cytidine					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_14902_s_116	10329690	Uracil was selected as the base because RNase-4, one of the targets for the inhibitors under development (see below), strongly prefers this pyrimidine over cytosine ( 17), and most of the other mammalian RNases bind uridine and cytidine nucleotides with similar affinity ( 1,  23,  27).	transcription
57404	3	335392	7	NULL	NULL	0	NULL	statement 1			similar affinity to					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_21_14902_s_116	10329690	Uracil was selected as the base because RNase-4, one of the targets for the inhibitors under development (see below), strongly prefers this pyrimidine over cytosine ( 17), and most of the other mammalian RNases bind uridine and cytidine nucleotides with similar affinity ( 1,  23,  27).	transcription
78622	1	335393	6	NULL	NULL	0	NULL	APOBEC3	GP		is					apolipoprotein B-editing catalytic polypeptide 3	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_31_22161_s_27	16735504	As APOBEC3G, a member of the recently discovered human cytidine deaminase family named apolipoprotein B-editing catalytic polypeptide 3 (APOBEC3), deaminates cytosine residues to uracil in the growing minus strand viral DNA during retroviral reverse transcription, we wanted to evaluate whether members of the APOBEC3 family also interfere with L1 retrotransposition, which is also dependent on reverse transcription of template RNA.	transcription
78623	2	335393	6	NULL	NULL	0	NULL	APOBEC3	GP		belongs to					cytidine deaminase family		human			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_31_22161_s_27	16735504	As APOBEC3G, a member of the recently discovered human cytidine deaminase family named apolipoprotein B-editing catalytic polypeptide 3 (APOBEC3), deaminates cytosine residues to uracil in the growing minus strand viral DNA during retroviral reverse transcription, we wanted to evaluate whether members of the APOBEC3 family also interfere with L1 retrotransposition, which is also dependent on reverse transcription of template RNA.	transcription
78624	3	335393	6	NULL	NULL	0	NULL	cytosine			is converted to					Uracil					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_31_22161_s_27	16735504	As APOBEC3G, a member of the recently discovered human cytidine deaminase family named apolipoprotein B-editing catalytic polypeptide 3 (APOBEC3), deaminates cytosine residues to uracil in the growing minus strand viral DNA during retroviral reverse transcription, we wanted to evaluate whether members of the APOBEC3 family also interfere with L1 retrotransposition, which is also dependent on reverse transcription of template RNA.	transcription
78625	4	335393	6	NULL	NULL	0	NULL	statement 3	Process		occurs during					reverse transcription	Process	retroviral 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_31_22161_s_27	16735504	As APOBEC3G, a member of the recently discovered human cytidine deaminase family named apolipoprotein B-editing catalytic polypeptide 3 (APOBEC3), deaminates cytosine residues to uracil in the growing minus strand viral DNA during retroviral reverse transcription, we wanted to evaluate whether members of the APOBEC3 family also interfere with L1 retrotransposition, which is also dependent on reverse transcription of template RNA.	transcription
57405	1	335393	7	NULL	NULL	0	NULL	APOBEC3G			belongs to					cytidine deaminase family		human			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_31_22161_s_27	16735504	As APOBEC3G, a member of the recently discovered human cytidine deaminase family named apolipoprotein B-editing catalytic polypeptide 3 (APOBEC3), deaminates cytosine residues to uracil in the growing minus strand viral DNA during retroviral reverse transcription, we wanted to evaluate whether members of the APOBEC3 family also interfere with L1 retrotransposition, which is also dependent on reverse transcription of template RNA.	transcription
57406	2	335393	7	NULL	NULL	0	NULL	APOBEC3G			is					apolipoprotein B-editing catalytic polypeptide 3					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_31_22161_s_27	16735504	As APOBEC3G, a member of the recently discovered human cytidine deaminase family named apolipoprotein B-editing catalytic polypeptide 3 (APOBEC3), deaminates cytosine residues to uracil in the growing minus strand viral DNA during retroviral reverse transcription, we wanted to evaluate whether members of the APOBEC3 family also interfere with L1 retrotransposition, which is also dependent on reverse transcription of template RNA.	transcription
57407	3	335393	7	NULL	NULL	0	NULL	cytosine residues			deaminates to					uracil					NULL	growing minus strand viral DNA	0	NULL	NULL	NULL	gw70_jbiolchem_281_31_22161_s_27	16735504	As APOBEC3G, a member of the recently discovered human cytidine deaminase family named apolipoprotein B-editing catalytic polypeptide 3 (APOBEC3), deaminates cytosine residues to uracil in the growing minus strand viral DNA during retroviral reverse transcription, we wanted to evaluate whether members of the APOBEC3 family also interfere with L1 retrotransposition, which is also dependent on reverse transcription of template RNA.	transcription
57408	4	335393	7	NULL	NULL	0	NULL	APOBEC3			deaminates 					statement 3					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_31_22161_s_27	16735504	As APOBEC3G, a member of the recently discovered human cytidine deaminase family named apolipoprotein B-editing catalytic polypeptide 3 (APOBEC3), deaminates cytosine residues to uracil in the growing minus strand viral DNA during retroviral reverse transcription, we wanted to evaluate whether members of the APOBEC3 family also interfere with L1 retrotransposition, which is also dependent on reverse transcription of template RNA.	transcription
57409	5	335393	7	NULL	NULL	0	NULL	statement 3			during					retroviral reverse transcription					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_31_22161_s_27	16735504	As APOBEC3G, a member of the recently discovered human cytidine deaminase family named apolipoprotein B-editing catalytic polypeptide 3 (APOBEC3), deaminates cytosine residues to uracil in the growing minus strand viral DNA during retroviral reverse transcription, we wanted to evaluate whether members of the APOBEC3 family also interfere with L1 retrotransposition, which is also dependent on reverse transcription of template RNA.	transcription
57410	6	335393	7	NULL	NULL	0	NULL	L1 retrotransposition			depends on					template RNA		 reverse transcription of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_31_22161_s_27	16735504	As APOBEC3G, a member of the recently discovered human cytidine deaminase family named apolipoprotein B-editing catalytic polypeptide 3 (APOBEC3), deaminates cytosine residues to uracil in the growing minus strand viral DNA during retroviral reverse transcription, we wanted to evaluate whether members of the APOBEC3 family also interfere with L1 retrotransposition, which is also dependent on reverse transcription of template RNA.	transcription
78617	1	335395	6	NULL	NULL	0	NULL	L-tyrosine	AminoAcid		is converted to					L-dopa	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21225_s_235	16714291	The conversion of L-tyrosine to L-dopa by TH is the rate-limiting step for catecholamine biosynthesis ( ,  ), and PNMT catalyzes the synthesis of epinephrine from nor epinephrine ( ) ( Fig. 7 A).	transcription
78618	2	335395	6	NULL	NULL	0	NULL	TH	GP		performs					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21225_s_235	16714291	The conversion of L-tyrosine to L-dopa by TH is the rate-limiting step for catecholamine biosynthesis ( ,  ), and PNMT catalyzes the synthesis of epinephrine from nor epinephrine ( ) ( Fig. 7 A).	transcription
78619	3	335395	6	NULL	NULL	0	NULL	statement 1	Process		is a step for					catecholamine	Chemical	biosynthesis of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21225_s_235	16714291	The conversion of L-tyrosine to L-dopa by TH is the rate-limiting step for catecholamine biosynthesis ( ,  ), and PNMT catalyzes the synthesis of epinephrine from nor epinephrine ( ) ( Fig. 7 A).	transcription
78620	4	335395	6	NULL	NULL	0	NULL	nor epinephrine	Chemical		is converted to					epinephrine	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21225_s_235	16714291	The conversion of L-tyrosine to L-dopa by TH is the rate-limiting step for catecholamine biosynthesis ( ,  ), and PNMT catalyzes the synthesis of epinephrine from nor epinephrine ( ) ( Fig. 7 A).	transcription
78621	5	335395	6	NULL	NULL	0	NULL	PNMT	GP		catalyzes					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21225_s_235	16714291	The conversion of L-tyrosine to L-dopa by TH is the rate-limiting step for catecholamine biosynthesis ( ,  ), and PNMT catalyzes the synthesis of epinephrine from nor epinephrine ( ) ( Fig. 7 A).	transcription
57411	1	335395	7	NULL	NULL	0	NULL	 L-tyrosine			converted to					 L-dopa					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21225_s_235	16714291	The conversion of L-tyrosine to L-dopa by TH is the rate-limiting step for catecholamine biosynthesis ( ,  ), and PNMT catalyzes the synthesis of epinephrine from nor epinephrine ( ) ( Fig. 7 A).	transcription
57412	2	335395	7	NULL	NULL	0	NULL	TH			catalyze					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21225_s_235	16714291	The conversion of L-tyrosine to L-dopa by TH is the rate-limiting step for catecholamine biosynthesis ( ,  ), and PNMT catalyzes the synthesis of epinephrine from nor epinephrine ( ) ( Fig. 7 A).	transcription
57413	3	335395	7	NULL	NULL	0	NULL	statement 1			rate-limiting step for					catecholamine		biosynthesis of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21225_s_235	16714291	The conversion of L-tyrosine to L-dopa by TH is the rate-limiting step for catecholamine biosynthesis ( ,  ), and PNMT catalyzes the synthesis of epinephrine from nor epinephrine ( ) ( Fig. 7 A).	transcription
57414	4	335395	7	NULL	NULL	0	NULL	epinephrine			synthesized from					nor epinephrine					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21225_s_235	16714291	The conversion of L-tyrosine to L-dopa by TH is the rate-limiting step for catecholamine biosynthesis ( ,  ), and PNMT catalyzes the synthesis of epinephrine from nor epinephrine ( ) ( Fig. 7 A).	transcription
57415	5	335395	7	NULL	NULL	0	NULL	PNMT			catalyze					statement 4					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21225_s_235	16714291	The conversion of L-tyrosine to L-dopa by TH is the rate-limiting step for catecholamine biosynthesis ( ,  ), and PNMT catalyzes the synthesis of epinephrine from nor epinephrine ( ) ( Fig. 7 A).	transcription
78607	1	335396	6	NULL	NULL	0	NULL	thrombin	GP		stimulates					platelets	cell				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10941_s_40	9099753	Stimulation of platelets by several agonists including thrombin, collagen, ADP, epinephrine, and the calcium ionophore A23187 induced the tyrosine phosphorylation of RAFTK.	transcription
78608	2	335396	6	NULL	NULL	0	NULL	collagen	GP		stimulates					platelets	cell				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10941_s_40	9099753	Stimulation of platelets by several agonists including thrombin, collagen, ADP, epinephrine, and the calcium ionophore A23187 induced the tyrosine phosphorylation of RAFTK.	transcription
78609	3	335396	6	NULL	NULL	0	NULL	ADP	Chemical		stimulates					platelets	cell				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10941_s_40	9099753	Stimulation of platelets by several agonists including thrombin, collagen, ADP, epinephrine, and the calcium ionophore A23187 induced the tyrosine phosphorylation of RAFTK.	transcription
78610	4	335396	6	NULL	NULL	0	NULL	epinephrine	Chemical		stimulates					platelets	cell				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10941_s_40	9099753	Stimulation of platelets by several agonists including thrombin, collagen, ADP, epinephrine, and the calcium ionophore A23187 induced the tyrosine phosphorylation of RAFTK.	transcription
78611	5	335396	6	NULL	NULL	0	NULL	calcium ionophore A23187	Chemical		stimulates					platelets	cell				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10941_s_40	9099753	Stimulation of platelets by several agonists including thrombin, collagen, ADP, epinephrine, and the calcium ionophore A23187 induced the tyrosine phosphorylation of RAFTK.	transcription
78612	6	335396	6	NULL	NULL	0	NULL	thrombin	GP		induces					RAFTK	GP	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10941_s_40	9099753	Stimulation of platelets by several agonists including thrombin, collagen, ADP, epinephrine, and the calcium ionophore A23187 induced the tyrosine phosphorylation of RAFTK.	transcription
78613	7	335396	6	NULL	NULL	0	NULL	collagen	GP		induces					RAFTK	GP	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10941_s_40	9099753	Stimulation of platelets by several agonists including thrombin, collagen, ADP, epinephrine, and the calcium ionophore A23187 induced the tyrosine phosphorylation of RAFTK.	transcription
78614	8	335396	6	NULL	NULL	0	NULL	ADP	Chemical		induces					RAFTK	GP	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10941_s_40	9099753	Stimulation of platelets by several agonists including thrombin, collagen, ADP, epinephrine, and the calcium ionophore A23187 induced the tyrosine phosphorylation of RAFTK.	transcription
78615	9	335396	6	NULL	NULL	0	NULL	epinephrine	Chemical		induces					RAFTK	GP	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10941_s_40	9099753	Stimulation of platelets by several agonists including thrombin, collagen, ADP, epinephrine, and the calcium ionophore A23187 induced the tyrosine phosphorylation of RAFTK.	transcription
78616	10	335396	6	NULL	NULL	0	NULL	calcium ionophore A23187	Chemical		induces					RAFTK	GP	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10941_s_40	9099753	Stimulation of platelets by several agonists including thrombin, collagen, ADP, epinephrine, and the calcium ionophore A23187 induced the tyrosine phosphorylation of RAFTK.	transcription
57416	1	335396	7	NULL	NULL	0	NULL	thrombin			stimulates					platelets					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10941_s_40	9099753	Stimulation of platelets by several agonists including thrombin, collagen, ADP, epinephrine, and the calcium ionophore A23187 induced the tyrosine phosphorylation of RAFTK.	transcription
57417	2	335396	7	NULL	NULL	0	NULL	collagen			stimulates					platelets					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10941_s_40	9099753	Stimulation of platelets by several agonists including thrombin, collagen, ADP, epinephrine, and the calcium ionophore A23187 induced the tyrosine phosphorylation of RAFTK.	transcription
57418	3	335396	7	NULL	NULL	0	NULL	ADP			stimulates					platelets					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10941_s_40	9099753	Stimulation of platelets by several agonists including thrombin, collagen, ADP, epinephrine, and the calcium ionophore A23187 induced the tyrosine phosphorylation of RAFTK.	transcription
57419	4	335396	7	NULL	NULL	0	NULL	epinephrine			stimulates					platelets					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10941_s_40	9099753	Stimulation of platelets by several agonists including thrombin, collagen, ADP, epinephrine, and the calcium ionophore A23187 induced the tyrosine phosphorylation of RAFTK.	transcription
57420	5	335396	7	NULL	NULL	0	NULL	A23187 			stimulates					platelets					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10941_s_40	9099753	Stimulation of platelets by several agonists including thrombin, collagen, ADP, epinephrine, and the calcium ionophore A23187 induced the tyrosine phosphorylation of RAFTK.	transcription
57421	6	335396	7	NULL	NULL	0	NULL	statement 1			induce					RAFTK		phosphorylation of	tyrosine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10941_s_40	9099753	Stimulation of platelets by several agonists including thrombin, collagen, ADP, epinephrine, and the calcium ionophore A23187 induced the tyrosine phosphorylation of RAFTK.	transcription
57422	7	335396	7	NULL	NULL	0	NULL	statement 2			induce					RAFTK		phosphorylation of	tyrosine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10941_s_40	9099753	Stimulation of platelets by several agonists including thrombin, collagen, ADP, epinephrine, and the calcium ionophore A23187 induced the tyrosine phosphorylation of RAFTK.	transcription
57423	8	335396	7	NULL	NULL	0	NULL	statement 3			induce					RAFTK		phosphorylation of	tyrosine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10941_s_40	9099753	Stimulation of platelets by several agonists including thrombin, collagen, ADP, epinephrine, and the calcium ionophore A23187 induced the tyrosine phosphorylation of RAFTK.	transcription
57424	9	335396	7	NULL	NULL	0	NULL	statement 4			induce					RAFTK		phosphorylation of	tyrosine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10941_s_40	9099753	Stimulation of platelets by several agonists including thrombin, collagen, ADP, epinephrine, and the calcium ionophore A23187 induced the tyrosine phosphorylation of RAFTK.	transcription
57425	10	335396	7	NULL	NULL	0	NULL	statement 5			induce					RAFTK		phosphorylation of	tyrosine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10941_s_40	9099753	Stimulation of platelets by several agonists including thrombin, collagen, ADP, epinephrine, and the calcium ionophore A23187 induced the tyrosine phosphorylation of RAFTK.	transcription
57426	11	335396	7	NULL	NULL	0	NULL	A23187 			is a type of					calcium ionophore					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10941_s_40	9099753	Stimulation of platelets by several agonists including thrombin, collagen, ADP, epinephrine, and the calcium ionophore A23187 induced the tyrosine phosphorylation of RAFTK.	transcription
78516	1	335397	6	NULL	NULL	0	NULL	ADP			induces					beta3	GP	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_22_13878_s_95	9593734	Thus, ADP and ADP + epinephrine induced tyrosine phosphorylation of beta3 in an aggregation-dependent manner.	transcription
78517	2	335397	6	NULL	NULL	0	NULL	ADP + epinephrine	Chemical		induces					beta3	GP	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_22_13878_s_95	9593734	Thus, ADP and ADP + epinephrine induced tyrosine phosphorylation of beta3 in an aggregation-dependent manner.	transcription
57427	1	335397	7	NULL	NULL	0	NULL	ADP			induce					beta3		phosphorylation of	tyrosine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_22_13878_s_95	9593734	Thus, ADP and ADP + epinephrine induced tyrosine phosphorylation of beta3 in an aggregation-dependent manner.	transcription
57428	2	335397	7	NULL	NULL	0	NULL	ADP + epinephrine			induce					beta3		phosphorylation of	tyrosine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_22_13878_s_95	9593734	Thus, ADP and ADP + epinephrine induced tyrosine phosphorylation of beta3 in an aggregation-dependent manner.	transcription
57429	3	335397	7	NULL	NULL	0	NULL	statement 1			depends on					aggregation					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_22_13878_s_95	9593734	Thus, ADP and ADP + epinephrine induced tyrosine phosphorylation of beta3 in an aggregation-dependent manner.	transcription
57430	4	335397	7	NULL	NULL	0	NULL	statement 2			depends on					aggregation					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_22_13878_s_95	9593734	Thus, ADP and ADP + epinephrine induced tyrosine phosphorylation of beta3 in an aggregation-dependent manner.	transcription
78513	1	335398	6	NULL	NULL	0	NULL	thrombin	GP		induces					platelets	cell	aggregation of;; epinephrine-potentiated			NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-biochem-(tokyo)_121_2_9089407_s_1	9089407	Tyrosine phosphorylation and Syk activation are involved in thrombin-induced aggregation of epinephrine-potentiated platelets..	transcription
78514	2	335398	6	NULL	NULL	0	NULL	Tyrosine	AminoAcid	phosphorylation of	is involved in					statement 1	Process				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-biochem-(tokyo)_121_2_9089407_s_1	9089407	Tyrosine phosphorylation and Syk activation are involved in thrombin-induced aggregation of epinephrine-potentiated platelets..	transcription
78515	3	335398	6	NULL	NULL	0	NULL	Syk	GP	activation of	is involved in					statement 1	Process				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-biochem-(tokyo)_121_2_9089407_s_1	9089407	Tyrosine phosphorylation and Syk activation are involved in thrombin-induced aggregation of epinephrine-potentiated platelets..	transcription
57431	1	335398	7	NULL	NULL	0	NULL	epinephrine			potentiate					platelets					NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-biochem-(tokyo)_121_2_9089407_s_1	9089407	Tyrosine phosphorylation and Syk activation are involved in thrombin-induced aggregation of epinephrine-potentiated platelets..	transcription
57432	2	335398	7	NULL	NULL	0	NULL	thrombin			induce					statement 1		aggregation of 			NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-biochem-(tokyo)_121_2_9089407_s_1	9089407	Tyrosine phosphorylation and Syk activation are involved in thrombin-induced aggregation of epinephrine-potentiated platelets..	transcription
57433	3	335398	7	NULL	NULL	0	NULL			phosphorylation of	is involved in			tyrosine		statement 2					NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-biochem-(tokyo)_121_2_9089407_s_1	9089407	Tyrosine phosphorylation and Syk activation are involved in thrombin-induced aggregation of epinephrine-potentiated platelets..	transcription
57434	4	335398	7	NULL	NULL	0	NULL	Syk		activation of	is involved in					statement 2					NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-biochem-(tokyo)_121_2_9089407_s_1	9089407	Tyrosine phosphorylation and Syk activation are involved in thrombin-induced aggregation of epinephrine-potentiated platelets..	transcription
78509	1	335399	6	NULL	NULL	0	NULL	epinephrine	Chemical		phosphorylates					Insulin receptor	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_5_3254_s_257	14602724	Preincubation with sodium vanadate, an inhibitor of protein-tyrosine phosphatases, partially reversed the effects of epinephrine on the tyrosine phosphorylation of the insulin receptor ( Fig. 8 D).	transcription
78512	2	335399	6	NULL	NULL	0	NULL	sodium vanadate	Chemical		reverses					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_5_3254_s_257	14602724	Preincubation with sodium vanadate, an inhibitor of protein-tyrosine phosphatases, partially reversed the effects of epinephrine on the tyrosine phosphorylation of the insulin receptor ( Fig. 8 D).	transcription
57435	1	335399	7	NULL	NULL	0	NULL	epinephrine 			effect					insulin receptor		phosphorylation of	tyrosine		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_5_3254_s_257	14602724	Preincubation with sodium vanadate, an inhibitor of protein-tyrosine phosphatases, partially reversed the effects of epinephrine on the tyrosine phosphorylation of the insulin receptor ( Fig. 8 D).	transcription
57436	2	335399	7	NULL	NULL	0	NULL	sodium vanadate			reverse		partially			statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_5_3254_s_257	14602724	Preincubation with sodium vanadate, an inhibitor of protein-tyrosine phosphatases, partially reversed the effects of epinephrine on the tyrosine phosphorylation of the insulin receptor ( Fig. 8 D).	transcription
57437	3	335399	7	NULL	NULL	0	NULL	sodium vanadate			is an inhibitor of					 protein-tyrosine phosphatases					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_5_3254_s_257	14602724	Preincubation with sodium vanadate, an inhibitor of protein-tyrosine phosphatases, partially reversed the effects of epinephrine on the tyrosine phosphorylation of the insulin receptor ( Fig. 8 D).	transcription
78505	1	335400	6	NULL	NULL	0	NULL	epinephrine	Chemical		induces					tyrosine	AminoAcid	phosphorylation of			NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-biochem-(tokyo)_121_2_9089407_s_5	9089407	Although  epinephrine alone (4 microM) slightly induced protein-tyrosine phosphorylation  and Syk activation, the presence of epinephrine caused a shift to the  left in the dose-dependence of thrombin (0.01-0.5 U/ml)-induced tyrosine  phosphorylation and Syk activation, as well as platelet aggregation.	transcription
78506	2	335400	6	NULL	NULL	0	NULL	epinephrine	Chemical		induces					Syk	GP	activation of 			NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-biochem-(tokyo)_121_2_9089407_s_5	9089407	Although  epinephrine alone (4 microM) slightly induced protein-tyrosine phosphorylation  and Syk activation, the presence of epinephrine caused a shift to the  left in the dose-dependence of thrombin (0.01-0.5 U/ml)-induced tyrosine  phosphorylation and Syk activation, as well as platelet aggregation.	transcription
78507	3	335400	6	NULL	NULL	0	NULL	epinephrine	Chemical		induces					platelet aggregation 	Process				NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-biochem-(tokyo)_121_2_9089407_s_5	9089407	Although  epinephrine alone (4 microM) slightly induced protein-tyrosine phosphorylation  and Syk activation, the presence of epinephrine caused a shift to the  left in the dose-dependence of thrombin (0.01-0.5 U/ml)-induced tyrosine  phosphorylation and Syk activation, as well as platelet aggregation.	transcription
57438	1	335400	7	NULL	NULL	0	NULL	epinephrine			induce		slightly			protein-tyrosine		phosphorylation of			NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-biochem-(tokyo)_121_2_9089407_s_5	9089407	Although  epinephrine alone (4 microM) slightly induced protein-tyrosine phosphorylation  and Syk activation, the presence of epinephrine caused a shift to the  left in the dose-dependence of thrombin (0.01-0.5 U/ml)-induced tyrosine  phosphorylation and Syk activation, as well as platelet aggregation.	transcription
57439	2	335400	7	NULL	NULL	0	NULL	epinephrine			induce		slightly			Syk		activation of			NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-biochem-(tokyo)_121_2_9089407_s_5	9089407	Although  epinephrine alone (4 microM) slightly induced protein-tyrosine phosphorylation  and Syk activation, the presence of epinephrine caused a shift to the  left in the dose-dependence of thrombin (0.01-0.5 U/ml)-induced tyrosine  phosphorylation and Syk activation, as well as platelet aggregation.	transcription
57440	3	335400	7	NULL	NULL	0	NULL	thrombin			induce							phosphorylation of	tyrosine		NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-biochem-(tokyo)_121_2_9089407_s_5	9089407	Although  epinephrine alone (4 microM) slightly induced protein-tyrosine phosphorylation  and Syk activation, the presence of epinephrine caused a shift to the  left in the dose-dependence of thrombin (0.01-0.5 U/ml)-induced tyrosine  phosphorylation and Syk activation, as well as platelet aggregation.	transcription
57441	4	335400	7	NULL	NULL	0	NULL	thrombin			induce					Syk		activation of			NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-biochem-(tokyo)_121_2_9089407_s_5	9089407	Although  epinephrine alone (4 microM) slightly induced protein-tyrosine phosphorylation  and Syk activation, the presence of epinephrine caused a shift to the  left in the dose-dependence of thrombin (0.01-0.5 U/ml)-induced tyrosine  phosphorylation and Syk activation, as well as platelet aggregation.	transcription
57442	5	335400	7	NULL	NULL	0	NULL	thrombin			induce					platelet		aggregation of 			NULL		0	NULL	NULL	NULL	abs-batch0620-0649_j-biochem-(tokyo)_121_2_9089407_s_5	9089407	Although  epinephrine alone (4 microM) slightly induced protein-tyrosine phosphorylation  and Syk activation, the presence of epinephrine caused a shift to the  left in the dose-dependence of thrombin (0.01-0.5 U/ml)-induced tyrosine  phosphorylation and Syk activation, as well as platelet aggregation.	transcription
78736	1	335401	6	NULL	NULL	NULL	NULL	angiotensin II	GP		stimulates					p120/p125	GP	phosphorylation of;; tyrosine			NULL	liver endothelial cells	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_314_3_916_s_219	14741724	A similar finding was made in liver endothelial cells, in which  angiotensin II, vasopressin, and epinephrine stimulated tyrosine phosphorylation  of p120/125, p75/p78, and p66 proteins [ 2.	transcription
78737	2	335401	6	NULL	NULL	NULL	NULL	vasopressin	GP		stimulates					p75/p78	GP	phosphorylation of;; tyrosine			NULL	liver endothelial cells	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_314_3_916_s_219	14741724	A similar finding was made in liver endothelial cells, in which  angiotensin II, vasopressin, and epinephrine stimulated tyrosine phosphorylation  of p120/125, p75/p78, and p66 proteins [ 2.	transcription
78738	3	335401	6	NULL	NULL	0	NULL	epinephrine	GP		stimulates					p66	GP	phosphorylation of;; tyrosine			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_314_3_916_s_219	14741724	A similar finding was made in liver endothelial cells, in which  angiotensin II, vasopressin, and epinephrine stimulated tyrosine phosphorylation  of p120/125, p75/p78, and p66 proteins [ 2.	transcription
57443	1	335401	7	NULL	NULL	0	NULL	 angiotensin II			stimulate					p120/125		phosphorylation of 	tyrosine		NULL	liver endothelial cells	0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_314_3_916_s_219	14741724	A similar finding was made in liver endothelial cells, in which  angiotensin II, vasopressin, and epinephrine stimulated tyrosine phosphorylation  of p120/125, p75/p78, and p66 proteins [ 2.	transcription
57444	2	335401	7	NULL	NULL	0	NULL	angiotensin II			stimulate					 p75/p78		phosphorylation of	tyrosine		NULL	liver endothelial cells	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_314_3_916_s_219	14741724	A similar finding was made in liver endothelial cells, in which  angiotensin II, vasopressin, and epinephrine stimulated tyrosine phosphorylation  of p120/125, p75/p78, and p66 proteins [ 2.	transcription
57445	3	335401	7	NULL	NULL	0	NULL	angiotensin II			stimulate					p66 protein		phosphorylation of	tyrosine		NULL	liver endothelial cells	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_314_3_916_s_219	14741724	A similar finding was made in liver endothelial cells, in which  angiotensin II, vasopressin, and epinephrine stimulated tyrosine phosphorylation  of p120/125, p75/p78, and p66 proteins [ 2.	transcription
57446	4	335401	7	NULL	NULL	0	NULL	vasopressin			stimulate					p120/125		phosphorylation of	tyrosine		NULL	liver endothelial cells	0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_314_3_916_s_219	14741724	A similar finding was made in liver endothelial cells, in which  angiotensin II, vasopressin, and epinephrine stimulated tyrosine phosphorylation  of p120/125, p75/p78, and p66 proteins [ 2.	transcription
57447	5	335401	7	NULL	NULL	0	NULL	vasopressin			stimulate					p75/p78		phosphorylation of	tyrosine		NULL	liver endothelial cells	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_314_3_916_s_219	14741724	A similar finding was made in liver endothelial cells, in which  angiotensin II, vasopressin, and epinephrine stimulated tyrosine phosphorylation  of p120/125, p75/p78, and p66 proteins [ 2.	transcription
57448	6	335401	7	NULL	NULL	0	NULL	vasopressin			stimulate					p66 protein		phosphorylation of	tyrosine		NULL	liver endothelial cells	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_314_3_916_s_219	14741724	A similar finding was made in liver endothelial cells, in which  angiotensin II, vasopressin, and epinephrine stimulated tyrosine phosphorylation  of p120/125, p75/p78, and p66 proteins [ 2.	transcription
57449	7	335401	7	NULL	NULL	0	NULL	epinephrine			stimulate					p120/125		phosphorylation of	tyrosine		NULL	liver endothelial cells	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_314_3_916_s_219	14741724	A similar finding was made in liver endothelial cells, in which  angiotensin II, vasopressin, and epinephrine stimulated tyrosine phosphorylation  of p120/125, p75/p78, and p66 proteins [ 2.	transcription
57450	8	335401	7	NULL	NULL	0	NULL	epinephrine			stimulate					p75/p78		phosphorylation of	tyrosine		NULL	liver endothelial cells	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_314_3_916_s_219	14741724	A similar finding was made in liver endothelial cells, in which  angiotensin II, vasopressin, and epinephrine stimulated tyrosine phosphorylation  of p120/125, p75/p78, and p66 proteins [ 2.	transcription
57451	9	335401	7	NULL	NULL	0	NULL	epinephrine			stimulate					p66 protein		phosphorylation of	tyrosine		NULL	liver endothelial cells	NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_314_3_916_s_219	14741724	A similar finding was made in liver endothelial cells, in which  angiotensin II, vasopressin, and epinephrine stimulated tyrosine phosphorylation  of p120/125, p75/p78, and p66 proteins [ 2.	transcription
78739	1	335402	6	NULL	NULL	0	NULL	insulin	GP		induces					IRS-1	GP	phosphorylation of	tyrosine		NULL		0	NULL	NULL	NULL	gw60_febslett_421_3_191_s_172	9468304	We have shown that chronic GH or acute epinephrine treatment can specifically decrease insulin-induced IRS-1 tyrosine phosphorylation and association with PI 3-kinase.	transcription
78740	2	335402	6	NULL	NULL	0	NULL	epinephrine	GP		decrease					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_421_3_191_s_172	9468304	We have shown that chronic GH or acute epinephrine treatment can specifically decrease insulin-induced IRS-1 tyrosine phosphorylation and association with PI 3-kinase.	transcription
78741	3	335402	6	NULL	NULL	0	NULL	GH	GP		decreases					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_421_3_191_s_172	9468304	We have shown that chronic GH or acute epinephrine treatment can specifically decrease insulin-induced IRS-1 tyrosine phosphorylation and association with PI 3-kinase.	transcription
57452	1	335402	7	NULL	NULL	0	NULL	insulin			induce					IRS-1		phosphorylation of	tyrosine		NULL		0	NULL	NULL	NULL	gw60_febslett_421_3_191_s_172	9468304	We have shown that chronic GH or acute epinephrine treatment can specifically decrease insulin-induced IRS-1 tyrosine phosphorylation and association with PI 3-kinase.	transcription
57453	2	335402	7	NULL	NULL	0	NULL	insulin			induce					PI 3-kinase		association with			NULL		0	NULL	NULL	NULL	gw60_febslett_421_3_191_s_172	9468304	We have shown that chronic GH or acute epinephrine treatment can specifically decrease insulin-induced IRS-1 tyrosine phosphorylation and association with PI 3-kinase.	transcription
57454	3	335402	7	NULL	NULL	0	NULL	chronic GH		treatment with	decrease		specifically			statement 1					NULL		NULL	NULL	NULL	NULL	gw60_febslett_421_3_191_s_172	9468304	We have shown that chronic GH or acute epinephrine treatment can specifically decrease insulin-induced IRS-1 tyrosine phosphorylation and association with PI 3-kinase.	transcription
57455	4	335402	7	NULL	NULL	0	NULL	chronic GH		treatment with	decrease		specifically			statement 2					NULL		NULL	NULL	NULL	NULL	gw60_febslett_421_3_191_s_172	9468304	We have shown that chronic GH or acute epinephrine treatment can specifically decrease insulin-induced IRS-1 tyrosine phosphorylation and association with PI 3-kinase.	transcription
57456	5	335402	7	NULL	NULL	0	NULL	acute epinephrine 		treatment with	decrease		specifically			statement 1					NULL		NULL	NULL	NULL	NULL	gw60_febslett_421_3_191_s_172	9468304	We have shown that chronic GH or acute epinephrine treatment can specifically decrease insulin-induced IRS-1 tyrosine phosphorylation and association with PI 3-kinase.	transcription
57457	6	335402	7	NULL	NULL	0	NULL	acute epinephrine 		treatment with	decrease		specifically			statement 2					NULL		0	NULL	NULL	NULL	gw60_febslett_421_3_191_s_172	9468304	We have shown that chronic GH or acute epinephrine treatment can specifically decrease insulin-induced IRS-1 tyrosine phosphorylation and association with PI 3-kinase.	transcription
78742	1	335403	6	NULL	NULL	0	NULL	ST	Chemical		induces					Myocyte 	Cell	apoptosis of 			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_58_6_1546_s_109	11093795	Tyrosine-kinase inhibition by 50 muM genistein blunted the protective effects of 0.1 muM epinephrine and serum against ST-induced myocyte apoptosis.	transcription
78743	2	335403	6	NULL	NULL	NULL	NULL	epinephrine	Chemical		protects					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_58_6_1546_s_109	11093795	Tyrosine-kinase inhibition by 50 muM genistein blunted the protective effects of 0.1 muM epinephrine and serum against ST-induced myocyte apoptosis.	transcription
78744	3	335403	6	NULL	NULL	0	NULL	serum	CellComponent		protects					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_58_6_1546_s_109	11093795	Tyrosine-kinase inhibition by 50 muM genistein blunted the protective effects of 0.1 muM epinephrine and serum against ST-induced myocyte apoptosis.	transcription
78745	4	335403	6	NULL	NULL	0	NULL	genistein	Chemical		inhibits					tyrosine kinase	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_58_6_1546_s_109	11093795	Tyrosine-kinase inhibition by 50 muM genistein blunted the protective effects of 0.1 muM epinephrine and serum against ST-induced myocyte apoptosis.	transcription
78746	5	335403	6	NULL	NULL	0	NULL	statement 4	Process		blunts					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_58_6_1546_s_109	11093795	Tyrosine-kinase inhibition by 50 muM genistein blunted the protective effects of 0.1 muM epinephrine and serum against ST-induced myocyte apoptosis.	transcription
78747	6	335403	6	NULL	NULL	0	NULL	statement 4	Process		blunts					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_58_6_1546_s_109	11093795	Tyrosine-kinase inhibition by 50 muM genistein blunted the protective effects of 0.1 muM epinephrine and serum against ST-induced myocyte apoptosis.	transcription
57458	1	335403	7	NULL	NULL	0	NULL	genistein			inhibits					Tyrosine-kinase					NULL		0	NULL	NULL	NULL	gw60_molpharmacol_58_6_1546_s_109	11093795	Tyrosine-kinase inhibition by 50 muM genistein blunted the protective effects of 0.1 muM epinephrine and serum against ST-induced myocyte apoptosis.	transcription
57459	2	335403	7	NULL	NULL	0	NULL	ST			induce					myocyte 		apoptosis of			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_58_6_1546_s_109	11093795	Tyrosine-kinase inhibition by 50 muM genistein blunted the protective effects of 0.1 muM epinephrine and serum against ST-induced myocyte apoptosis.	transcription
57460	3	335403	7	NULL	NULL	0	NULL	epinephrine 			protects					statement 2					NULL		0	NULL	NULL	NULL	gw60_molpharmacol_58_6_1546_s_109	11093795	Tyrosine-kinase inhibition by 50 muM genistein blunted the protective effects of 0.1 muM epinephrine and serum against ST-induced myocyte apoptosis.	transcription
57461	4	335403	7	NULL	NULL	0	NULL	serum			protects					statement 2					NULL		0	NULL	NULL	NULL	gw60_molpharmacol_58_6_1546_s_109	11093795	Tyrosine-kinase inhibition by 50 muM genistein blunted the protective effects of 0.1 muM epinephrine and serum against ST-induced myocyte apoptosis.	transcription
57462	5	335403	7	NULL	NULL	0	NULL	statement 1			blunts					statement 3					NULL		0	NULL	NULL	NULL	gw60_molpharmacol_58_6_1546_s_109	11093795	Tyrosine-kinase inhibition by 50 muM genistein blunted the protective effects of 0.1 muM epinephrine and serum against ST-induced myocyte apoptosis.	transcription
57463	6	335403	7	NULL	NULL	0	NULL	statement 1			blunts					statement 4					NULL		0	NULL	NULL	NULL	gw60_molpharmacol_58_6_1546_s_109	11093795	Tyrosine-kinase inhibition by 50 muM genistein blunted the protective effects of 0.1 muM epinephrine and serum against ST-induced myocyte apoptosis.	transcription
78748	1	335404	6	NULL	NULL	0	NULL	ST	Chemical		induces					cardiac myocytes	cell	adult, apoptosis of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_58_6_1546_s_123	11093795	Altogether, these results suggested that the protective effect of epinephrine and serum on ST-induced apoptosis of adult cardiac myocytes could involve tyrosine-kinase-mediated ERK activation.	transcription
78749	2	335404	6	NULL	NULL	0	NULL	serum	CellComponent		protects					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_58_6_1546_s_123	11093795	Altogether, these results suggested that the protective effect of epinephrine and serum on ST-induced apoptosis of adult cardiac myocytes could involve tyrosine-kinase-mediated ERK activation.	transcription
78750	3	335404	6	NULL	NULL	0	NULL	epinephrine	Chemical		protects					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_58_6_1546_s_123	11093795	Altogether, these results suggested that the protective effect of epinephrine and serum on ST-induced apoptosis of adult cardiac myocytes could involve tyrosine-kinase-mediated ERK activation.	transcription
78751	4	335404	6	NULL	NULL	0	NULL	Tyrosine kinase	GP		mediates					ERK	GP	activation of 			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_58_6_1546_s_123	11093795	Altogether, these results suggested that the protective effect of epinephrine and serum on ST-induced apoptosis of adult cardiac myocytes could involve tyrosine-kinase-mediated ERK activation.	transcription
78752	5	335404	6	NULL	NULL	0	NULL	statement 2	Process		involve		could			statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_58_6_1546_s_123	11093795	Altogether, these results suggested that the protective effect of epinephrine and serum on ST-induced apoptosis of adult cardiac myocytes could involve tyrosine-kinase-mediated ERK activation.	transcription
78753	6	335404	6	NULL	NULL	0	NULL	statement 3	Process		involve		could			statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_58_6_1546_s_123	11093795	Altogether, these results suggested that the protective effect of epinephrine and serum on ST-induced apoptosis of adult cardiac myocytes could involve tyrosine-kinase-mediated ERK activation.	transcription
57464	1	335404	7	NULL	NULL	0	NULL	ST			induce					cardiac myocytes		apoptosis of adult			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_58_6_1546_s_123	11093795	Altogether, these results suggested that the protective effect of epinephrine and serum on ST-induced apoptosis of adult cardiac myocytes could involve tyrosine-kinase-mediated ERK activation.	transcription
57465	2	335404	7	NULL	NULL	0	NULL	tyrosine-kinase			mediates					ERK		activation of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_58_6_1546_s_123	11093795	Altogether, these results suggested that the protective effect of epinephrine and serum on ST-induced apoptosis of adult cardiac myocytes could involve tyrosine-kinase-mediated ERK activation.	transcription
57466	3	335404	7	NULL	NULL	0	NULL	epinephrine			protects					statement 1					NULL		0	NULL	NULL	NULL	gw60_molpharmacol_58_6_1546_s_123	11093795	Altogether, these results suggested that the protective effect of epinephrine and serum on ST-induced apoptosis of adult cardiac myocytes could involve tyrosine-kinase-mediated ERK activation.	transcription
57467	4	335404	7	NULL	NULL	0	NULL	serum			protects					statement 1					NULL		0	NULL	NULL	NULL	gw60_molpharmacol_58_6_1546_s_123	11093795	Altogether, these results suggested that the protective effect of epinephrine and serum on ST-induced apoptosis of adult cardiac myocytes could involve tyrosine-kinase-mediated ERK activation.	transcription
57468	5	335404	7	NULL	NULL	0	NULL	statement 1			involves					statement 2					NULL		0	NULL	NULL	NULL	gw60_molpharmacol_58_6_1546_s_123	11093795	Altogether, these results suggested that the protective effect of epinephrine and serum on ST-induced apoptosis of adult cardiac myocytes could involve tyrosine-kinase-mediated ERK activation.	transcription
78754	1	335405	6	NULL	NULL	0	NULL	Tyrosine hydroxylase 1	GP		is					TH 1	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_35_26683_s_11	10842166	The first and major rate-limiting regulatory step in the biosynthesis of the catecholamines (dopamine, norepinephrine, and epinephrine) is catalyzed by tyrosine hydroxylase (TH)1 ( 1).	transcription
78755	2	335405	6	NULL	NULL	0	NULL	dopamine	Chemical		is a type of					catecholamine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_35_26683_s_11	10842166	The first and major rate-limiting regulatory step in the biosynthesis of the catecholamines (dopamine, norepinephrine, and epinephrine) is catalyzed by tyrosine hydroxylase (TH)1 ( 1).	transcription
78757	3	335405	6	NULL	NULL	0	NULL	norepinephrine	Chemical		is a type of					catecholamine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_35_26683_s_11	10842166	The first and major rate-limiting regulatory step in the biosynthesis of the catecholamines (dopamine, norepinephrine, and epinephrine) is catalyzed by tyrosine hydroxylase (TH)1 ( 1).	transcription
78758	4	335405	6	NULL	NULL	0	NULL	epinephrine	Chemical		is a type of					catecholamine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_35_26683_s_11	10842166	The first and major rate-limiting regulatory step in the biosynthesis of the catecholamines (dopamine, norepinephrine, and epinephrine) is catalyzed by tyrosine hydroxylase (TH)1 ( 1).	transcription
78759	5	335405	6	NULL	NULL	0	NULL	TH 1	GP		catalyzes					dopamine	Chemical	biosynthesis of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_35_26683_s_11	10842166	The first and major rate-limiting regulatory step in the biosynthesis of the catecholamines (dopamine, norepinephrine, and epinephrine) is catalyzed by tyrosine hydroxylase (TH)1 ( 1).	transcription
78760	6	335405	6	NULL	NULL	NULL	NULL	TH 1	GP		catalyzes					norepinephrine	Chemical	biosynthesis of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_35_26683_s_11	10842166	The first and major rate-limiting regulatory step in the biosynthesis of the catecholamines (dopamine, norepinephrine, and epinephrine) is catalyzed by tyrosine hydroxylase (TH)1 ( 1).	transcription
78761	7	335405	6	NULL	NULL	0	NULL	TH 1	GP		catalyzes					epinephrine	Chemical	biosynthesis of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_35_26683_s_11	10842166	The first and major rate-limiting regulatory step in the biosynthesis of the catecholamines (dopamine, norepinephrine, and epinephrine) is catalyzed by tyrosine hydroxylase (TH)1 ( 1).	transcription
57469	1	335405	7	NULL	NULL	0	NULL	(TH)1			catalyze					dopamine		major rate-limiting regulatory step in biosynthesis of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_35_26683_s_11	10842166	The first and major rate-limiting regulatory step in the biosynthesis of the catecholamines (dopamine, norepinephrine, and epinephrine) is catalyzed by tyrosine hydroxylase (TH)1 ( 1).	transcription
57470	2	335405	7	NULL	NULL	0	NULL	(TH)1			catalyze					norepinephrine		major rate-limiting regulatory step in biosynthesis of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_35_26683_s_11	10842166	The first and major rate-limiting regulatory step in the biosynthesis of the catecholamines (dopamine, norepinephrine, and epinephrine) is catalyzed by tyrosine hydroxylase (TH)1 ( 1).	transcription
57471	3	335405	7	NULL	NULL	0	NULL	(TH)1			catalyze					epinephrine		major rate-limiting regulatory step in biosynthesis of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_35_26683_s_11	10842166	The first and major rate-limiting regulatory step in the biosynthesis of the catecholamines (dopamine, norepinephrine, and epinephrine) is catalyzed by tyrosine hydroxylase (TH)1 ( 1).	transcription
57472	4	335405	7	NULL	NULL	0	NULL	TH			is					tyrosine hydroxylase					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_35_26683_s_11	10842166	The first and major rate-limiting regulatory step in the biosynthesis of the catecholamines (dopamine, norepinephrine, and epinephrine) is catalyzed by tyrosine hydroxylase (TH)1 ( 1).	transcription
57473	5	335405	7	NULL	NULL	0	NULL	dopamine			is a type of					catecholamine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_35_26683_s_11	10842166	The first and major rate-limiting regulatory step in the biosynthesis of the catecholamines (dopamine, norepinephrine, and epinephrine) is catalyzed by tyrosine hydroxylase (TH)1 ( 1).	transcription
57474	6	335405	7	NULL	NULL	0	NULL	norepinephrine			is a type of					catecholamine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_35_26683_s_11	10842166	The first and major rate-limiting regulatory step in the biosynthesis of the catecholamines (dopamine, norepinephrine, and epinephrine) is catalyzed by tyrosine hydroxylase (TH)1 ( 1).	transcription
57475	7	335405	7	NULL	NULL	0	NULL	epinephrine 			is a type of					catecholamine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_35_26683_s_11	10842166	The first and major rate-limiting regulatory step in the biosynthesis of the catecholamines (dopamine, norepinephrine, and epinephrine) is catalyzed by tyrosine hydroxylase (TH)1 ( 1).	transcription
78762	1	335406	6	NULL	NULL	0	NULL	epinephrine receptor	GP		activates					adenylcyclase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_5226_s_260	9478978	The signal transduction pathway by which this is accomplished, involving transactivation of the EGF receptor and other tyrosine kinases, offers the opportunity for amplification of the signals and a prolonged response, much like the activation of adenylcyclase by the epinephrine receptor.	transcription
57476	1	335406	7	NULL	NULL	0	NULL	epinephrine receptor			activates					adenylcyclase					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_5226_s_260	9478978	The signal transduction pathway by which this is accomplished, involving transactivation of the EGF receptor and other tyrosine kinases, offers the opportunity for amplification of the signals and a prolonged response, much like the activation of adenylcyclase by the epinephrine receptor.	transcription
57477	2	335406	7	NULL	NULL	0	NULL	EGF receptor		transactivation of 	offers					amplification of signals		opportunity for			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_5226_s_260	9478978	The signal transduction pathway by which this is accomplished, involving transactivation of the EGF receptor and other tyrosine kinases, offers the opportunity for amplification of the signals and a prolonged response, much like the activation of adenylcyclase by the epinephrine receptor.	transcription
57478	3	335406	7	NULL	NULL	0	NULL	statement 2			leads to					prolonged response					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_5226_s_260	9478978	The signal transduction pathway by which this is accomplished, involving transactivation of the EGF receptor and other tyrosine kinases, offers the opportunity for amplification of the signals and a prolonged response, much like the activation of adenylcyclase by the epinephrine receptor.	transcription
78763	1	335407	6	NULL	NULL	0	NULL	thrombin	GP		induces					Vav	GP	phosphorylation of;; tyrosine			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_13_7544_s_88	8631786	Tyrosine Phosphorylation of Vav Is Induced by Thrombin  and Collagen, but Not by Other AgonistsIn order to determine if  other platelet agonists that work through G protein-coupled receptors  can cause Vav phosphorylation, we next stimulated platelets with either  U46619, epinephrine, or ADP. U46619 activates platelet TxA   receptors, epinephrine activates platelet  alpha -adrenergic receptors, and ADP is believed to activate  an unidentified purinergic receptor ( Fig. 3,  A  and  B).	transcription
78764	2	335407	6	NULL	NULL	0	NULL	collagen	GP		induces					Vav	GP	phosphorylation of;; tyrosine			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_13_7544_s_88	8631786	Tyrosine Phosphorylation of Vav Is Induced by Thrombin  and Collagen, but Not by Other AgonistsIn order to determine if  other platelet agonists that work through G protein-coupled receptors  can cause Vav phosphorylation, we next stimulated platelets with either  U46619, epinephrine, or ADP. U46619 activates platelet TxA   receptors, epinephrine activates platelet  alpha -adrenergic receptors, and ADP is believed to activate  an unidentified purinergic receptor ( Fig. 3,  A  and  B).	transcription
78765	3	335407	6	NULL	NULL	0	NULL	U46619	Chemical		activates					platelet TxA receptors	Cell				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_13_7544_s_88	8631786	Tyrosine Phosphorylation of Vav Is Induced by Thrombin  and Collagen, but Not by Other AgonistsIn order to determine if  other platelet agonists that work through G protein-coupled receptors  can cause Vav phosphorylation, we next stimulated platelets with either  U46619, epinephrine, or ADP. U46619 activates platelet TxA   receptors, epinephrine activates platelet  alpha -adrenergic receptors, and ADP is believed to activate  an unidentified purinergic receptor ( Fig. 3,  A  and  B).	transcription
78766	4	335407	6	NULL	NULL	0	NULL	epinephrine	GP		activates					platelet alpha -adrenergic receptor	cell				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_13_7544_s_88	8631786	Tyrosine Phosphorylation of Vav Is Induced by Thrombin  and Collagen, but Not by Other AgonistsIn order to determine if  other platelet agonists that work through G protein-coupled receptors  can cause Vav phosphorylation, we next stimulated platelets with either  U46619, epinephrine, or ADP. U46619 activates platelet TxA   receptors, epinephrine activates platelet  alpha -adrenergic receptors, and ADP is believed to activate  an unidentified purinergic receptor ( Fig. 3,  A  and  B).	transcription
57491	1	335407	7	NULL	NULL	0	NULL	Thrombin			induce					Vav		Phosphorylation of	tyrosine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_13_7544_s_88	8631786	Tyrosine Phosphorylation of Vav Is Induced by Thrombin  and Collagen, but Not by Other AgonistsIn order to determine if  other platelet agonists that work through G protein-coupled receptors  can cause Vav phosphorylation, we next stimulated platelets with either  U46619, epinephrine, or ADP. U46619 activates platelet TxA   receptors, epinephrine activates platelet  alpha -adrenergic receptors, and ADP is believed to activate  an unidentified purinergic receptor ( Fig. 3,  A  and  B).	transcription
57492	2	335407	7	NULL	NULL	0	NULL	collagen			induce					Vav		phosphorylation of	tyrosine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_13_7544_s_88	8631786	Tyrosine Phosphorylation of Vav Is Induced by Thrombin  and Collagen, but Not by Other AgonistsIn order to determine if  other platelet agonists that work through G protein-coupled receptors  can cause Vav phosphorylation, we next stimulated platelets with either  U46619, epinephrine, or ADP. U46619 activates platelet TxA   receptors, epinephrine activates platelet  alpha -adrenergic receptors, and ADP is believed to activate  an unidentified purinergic receptor ( Fig. 3,  A  and  B).	transcription
57493	3	335407	7	NULL	NULL	0	NULL	U46619			activates					TxA receptor		platelet			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_13_7544_s_88	8631786	Tyrosine Phosphorylation of Vav Is Induced by Thrombin  and Collagen, but Not by Other AgonistsIn order to determine if  other platelet agonists that work through G protein-coupled receptors  can cause Vav phosphorylation, we next stimulated platelets with either  U46619, epinephrine, or ADP. U46619 activates platelet TxA   receptors, epinephrine activates platelet  alpha -adrenergic receptors, and ADP is believed to activate  an unidentified purinergic receptor ( Fig. 3,  A  and  B).	transcription
57494	4	335407	7	NULL	NULL	0	NULL	epinephrine			activates					alpha -adrenergic receptor		platelet			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_13_7544_s_88	8631786	Tyrosine Phosphorylation of Vav Is Induced by Thrombin  and Collagen, but Not by Other AgonistsIn order to determine if  other platelet agonists that work through G protein-coupled receptors  can cause Vav phosphorylation, we next stimulated platelets with either  U46619, epinephrine, or ADP. U46619 activates platelet TxA   receptors, epinephrine activates platelet  alpha -adrenergic receptors, and ADP is believed to activate  an unidentified purinergic receptor ( Fig. 3,  A  and  B).	transcription
57495	5	335407	7	NULL	NULL	0	NULL	ADP			activates					unidentified purinergic receptor					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_13_7544_s_88	8631786	Tyrosine Phosphorylation of Vav Is Induced by Thrombin  and Collagen, but Not by Other AgonistsIn order to determine if  other platelet agonists that work through G protein-coupled receptors  can cause Vav phosphorylation, we next stimulated platelets with either  U46619, epinephrine, or ADP. U46619 activates platelet TxA   receptors, epinephrine activates platelet  alpha -adrenergic receptors, and ADP is believed to activate  an unidentified purinergic receptor ( Fig. 3,  A  and  B).	transcription
57502	1	335409	7	NULL	NULL	0	NULL	tyrosine			converted to					dopa					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_42_27051_s_60	9765218	We initially examined the functional role of V-1 in the regulation of expression of genes encoding TH ( 36), AADC ( 37), DBH ( 38), and PNMT ( 39,  40), which catalyze the four synthetic successive steps from tyrosine to dopa, dopamine, norepinephrine, and epinephrine.	transcription
57503	2	335409	7	NULL	NULL	0	NULL	TH 			catalyze					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_42_27051_s_60	9765218	We initially examined the functional role of V-1 in the regulation of expression of genes encoding TH ( 36), AADC ( 37), DBH ( 38), and PNMT ( 39,  40), which catalyze the four synthetic successive steps from tyrosine to dopa, dopamine, norepinephrine, and epinephrine.	transcription
57504	3	335409	7	NULL	NULL	0	NULL	dopa			converted to					dopamine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_42_27051_s_60	9765218	We initially examined the functional role of V-1 in the regulation of expression of genes encoding TH ( 36), AADC ( 37), DBH ( 38), and PNMT ( 39,  40), which catalyze the four synthetic successive steps from tyrosine to dopa, dopamine, norepinephrine, and epinephrine.	transcription
57505	4	335409	7	NULL	NULL	0	NULL	AADC			catalyze					statement 3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_42_27051_s_60	9765218	We initially examined the functional role of V-1 in the regulation of expression of genes encoding TH ( 36), AADC ( 37), DBH ( 38), and PNMT ( 39,  40), which catalyze the four synthetic successive steps from tyrosine to dopa, dopamine, norepinephrine, and epinephrine.	transcription
57506	5	335409	7	NULL	NULL	0	NULL	dopamine			converted to					norepinephrine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_42_27051_s_60	9765218	We initially examined the functional role of V-1 in the regulation of expression of genes encoding TH ( 36), AADC ( 37), DBH ( 38), and PNMT ( 39,  40), which catalyze the four synthetic successive steps from tyrosine to dopa, dopamine, norepinephrine, and epinephrine.	transcription
57507	6	335409	7	NULL	NULL	0	NULL	DBH			catalyze					statement 5					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_42_27051_s_60	9765218	We initially examined the functional role of V-1 in the regulation of expression of genes encoding TH ( 36), AADC ( 37), DBH ( 38), and PNMT ( 39,  40), which catalyze the four synthetic successive steps from tyrosine to dopa, dopamine, norepinephrine, and epinephrine.	transcription
57508	7	335409	7	NULL	NULL	0	NULL	norepinephrine			converted to					epinephrine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_42_27051_s_60	9765218	We initially examined the functional role of V-1 in the regulation of expression of genes encoding TH ( 36), AADC ( 37), DBH ( 38), and PNMT ( 39,  40), which catalyze the four synthetic successive steps from tyrosine to dopa, dopamine, norepinephrine, and epinephrine.	transcription
57509	8	335409	7	NULL	NULL	0	NULL	PNMT			catalyze					statement 7					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_42_27051_s_60	9765218	We initially examined the functional role of V-1 in the regulation of expression of genes encoding TH ( 36), AADC ( 37), DBH ( 38), and PNMT ( 39,  40), which catalyze the four synthetic successive steps from tyrosine to dopa, dopamine, norepinephrine, and epinephrine.	transcription
57510	9	335409	7	NULL	NULL	0	NULL	V-1 			regulates					TH gene		expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_42_27051_s_60	9765218	We initially examined the functional role of V-1 in the regulation of expression of genes encoding TH ( 36), AADC ( 37), DBH ( 38), and PNMT ( 39,  40), which catalyze the four synthetic successive steps from tyrosine to dopa, dopamine, norepinephrine, and epinephrine.	transcription
57511	10	335409	7	NULL	NULL	0	NULL	V-1			regulates					AADC gene		expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_42_27051_s_60	9765218	We initially examined the functional role of V-1 in the regulation of expression of genes encoding TH ( 36), AADC ( 37), DBH ( 38), and PNMT ( 39,  40), which catalyze the four synthetic successive steps from tyrosine to dopa, dopamine, norepinephrine, and epinephrine.	transcription
57512	11	335409	7	NULL	NULL	0	NULL	V-1 			regulates					DBH gene		expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_42_27051_s_60	9765218	We initially examined the functional role of V-1 in the regulation of expression of genes encoding TH ( 36), AADC ( 37), DBH ( 38), and PNMT ( 39,  40), which catalyze the four synthetic successive steps from tyrosine to dopa, dopamine, norepinephrine, and epinephrine.	transcription
57513	12	335409	7	NULL	NULL	0	NULL	V-1			regulates					PNMT gene		expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_42_27051_s_60	9765218	We initially examined the functional role of V-1 in the regulation of expression of genes encoding TH ( 36), AADC ( 37), DBH ( 38), and PNMT ( 39,  40), which catalyze the four synthetic successive steps from tyrosine to dopa, dopamine, norepinephrine, and epinephrine.	transcription
78773	1	335410	6	NULL	NULL	0	NULL	catecholamine	Chemical		response to					hypoglycemia	MedicalFinding				NULL		0	NULL	NULL	NULL	gw70_diabetes_54_12_3592_s_131	16306382	Assuming that the catecholamine biosynthetic enzyme protein and enzymatic activities paralleled the mRNA levels and that the reduced biosynthetic enzyme activities were sufficient to reduce adrenomedullary catecholamine contents, these data are consistent with the hypotheses that  1) reduced tyrosine hydroxylase activity contributes to reduced catecholamine responses to hypoglycemia in diabetes and  2) reduced phenylethanolamine  N-methyltransferase activity contributes to further reduced epinephrine responses to hypoglycemia following recent hypoglycemia.	transcription
78774	2	335410	6	NULL	NULL	0	NULL	tyrosine hydroxylase activity 	Process	reduction of 	contributes to					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_diabetes_54_12_3592_s_131	16306382	Assuming that the catecholamine biosynthetic enzyme protein and enzymatic activities paralleled the mRNA levels and that the reduced biosynthetic enzyme activities were sufficient to reduce adrenomedullary catecholamine contents, these data are consistent with the hypotheses that  1) reduced tyrosine hydroxylase activity contributes to reduced catecholamine responses to hypoglycemia in diabetes and  2) reduced phenylethanolamine  N-methyltransferase activity contributes to further reduced epinephrine responses to hypoglycemia following recent hypoglycemia.	transcription
78775	3	335410	6	NULL	NULL	0	NULL	epinephrine	Chemical		is responsive to					hypoglycemia	MedicalFinding				NULL		0	NULL	NULL	NULL	gw70_diabetes_54_12_3592_s_131	16306382	Assuming that the catecholamine biosynthetic enzyme protein and enzymatic activities paralleled the mRNA levels and that the reduced biosynthetic enzyme activities were sufficient to reduce adrenomedullary catecholamine contents, these data are consistent with the hypotheses that  1) reduced tyrosine hydroxylase activity contributes to reduced catecholamine responses to hypoglycemia in diabetes and  2) reduced phenylethanolamine  N-methyltransferase activity contributes to further reduced epinephrine responses to hypoglycemia following recent hypoglycemia.	transcription
78776	4	335410	6	NULL	NULL	0	NULL	phenylethanolamine N-methyltransferase activity	Process		contributes to					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_diabetes_54_12_3592_s_131	16306382	Assuming that the catecholamine biosynthetic enzyme protein and enzymatic activities paralleled the mRNA levels and that the reduced biosynthetic enzyme activities were sufficient to reduce adrenomedullary catecholamine contents, these data are consistent with the hypotheses that  1) reduced tyrosine hydroxylase activity contributes to reduced catecholamine responses to hypoglycemia in diabetes and  2) reduced phenylethanolamine  N-methyltransferase activity contributes to further reduced epinephrine responses to hypoglycemia following recent hypoglycemia.	transcription
57514	1	335410	7	NULL	NULL	0	NULL	tyrosine hydroxylase		reduced activity of	contributes to					catecholamine 		reduced response of			NULL		0	NULL	NULL	NULL	gw70_diabetes_54_12_3592_s_131	16306382	Assuming that the catecholamine biosynthetic enzyme protein and enzymatic activities paralleled the mRNA levels and that the reduced biosynthetic enzyme activities were sufficient to reduce adrenomedullary catecholamine contents, these data are consistent with the hypotheses that  1) reduced tyrosine hydroxylase activity contributes to reduced catecholamine responses to hypoglycemia in diabetes and  2) reduced phenylethanolamine  N-methyltransferase activity contributes to further reduced epinephrine responses to hypoglycemia following recent hypoglycemia.	transcription
57515	2	335410	7	NULL	NULL	0	NULL	statement 1			in response to					hypoglycemia					NULL	diabetes	NULL	NULL	NULL	NULL	gw70_diabetes_54_12_3592_s_131	16306382	Assuming that the catecholamine biosynthetic enzyme protein and enzymatic activities paralleled the mRNA levels and that the reduced biosynthetic enzyme activities were sufficient to reduce adrenomedullary catecholamine contents, these data are consistent with the hypotheses that  1) reduced tyrosine hydroxylase activity contributes to reduced catecholamine responses to hypoglycemia in diabetes and  2) reduced phenylethanolamine  N-methyltransferase activity contributes to further reduced epinephrine responses to hypoglycemia following recent hypoglycemia.	transcription
57516	3	335410	7	NULL	NULL	0	NULL	phenylethanolamine N-methyltransferase		reduced activity of	contribute to					epinephrine		reduced response of			NULL		0	NULL	NULL	NULL	gw70_diabetes_54_12_3592_s_131	16306382	Assuming that the catecholamine biosynthetic enzyme protein and enzymatic activities paralleled the mRNA levels and that the reduced biosynthetic enzyme activities were sufficient to reduce adrenomedullary catecholamine contents, these data are consistent with the hypotheses that  1) reduced tyrosine hydroxylase activity contributes to reduced catecholamine responses to hypoglycemia in diabetes and  2) reduced phenylethanolamine  N-methyltransferase activity contributes to further reduced epinephrine responses to hypoglycemia following recent hypoglycemia.	transcription
57517	4	335410	7	NULL	NULL	0	NULL	statement 3			in response to					hypoglycemia					NULL		0	NULL	NULL	NULL	gw70_diabetes_54_12_3592_s_131	16306382	Assuming that the catecholamine biosynthetic enzyme protein and enzymatic activities paralleled the mRNA levels and that the reduced biosynthetic enzyme activities were sufficient to reduce adrenomedullary catecholamine contents, these data are consistent with the hypotheses that  1) reduced tyrosine hydroxylase activity contributes to reduced catecholamine responses to hypoglycemia in diabetes and  2) reduced phenylethanolamine  N-methyltransferase activity contributes to further reduced epinephrine responses to hypoglycemia following recent hypoglycemia.	transcription
78777	1	335411	6	NULL	NULL	0	NULL	PKC	GP		induces					p125FAK	GP	phosphorylation of;; serine			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3044_s_33	10591686	Tyrosine phosphorylation of p125FAK in platelets stimulated with a mixture of epinephrine and anti-LIBS6 antibody 30  or in platelets adherent either to fibrinogen or to immobilized immunoglobulin IgG 31 32  is blocked when PKC activity was inhibited with a specific PKC inhibitor, bisindolylmaleimide GF 109203X, suggesting that p125FAK is activated downstream of PKC. PKC-induced serine phosphorylation of p125FAK has been suggested to regulate the intracellular stability of focal adhesion kinase in mouse 3T3 cells.	transcription
78778	2	335411	6	NULL	NULL	0	NULL	statement 1	Process		regulate					focal adhesion kinase	GP	intracellular stability of			NULL	mouse 3T3 cells	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3044_s_33	10591686	Tyrosine phosphorylation of p125FAK in platelets stimulated with a mixture of epinephrine and anti-LIBS6 antibody 30  or in platelets adherent either to fibrinogen or to immobilized immunoglobulin IgG 31 32  is blocked when PKC activity was inhibited with a specific PKC inhibitor, bisindolylmaleimide GF 109203X, suggesting that p125FAK is activated downstream of PKC. PKC-induced serine phosphorylation of p125FAK has been suggested to regulate the intracellular stability of focal adhesion kinase in mouse 3T3 cells.	transcription
78779	3	335411	6	NULL	NULL	0	NULL	p125FAK	GP		is activated					PKC	GP	downstream of 			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3044_s_33	10591686	Tyrosine phosphorylation of p125FAK in platelets stimulated with a mixture of epinephrine and anti-LIBS6 antibody 30  or in platelets adherent either to fibrinogen or to immobilized immunoglobulin IgG 31 32  is blocked when PKC activity was inhibited with a specific PKC inhibitor, bisindolylmaleimide GF 109203X, suggesting that p125FAK is activated downstream of PKC. PKC-induced serine phosphorylation of p125FAK has been suggested to regulate the intracellular stability of focal adhesion kinase in mouse 3T3 cells.	transcription
57518	1	335411	7	NULL	NULL	0	NULL	epinephrine			stimulate					 p125FAK		phosphorylation of	tyrosine		NULL	platelets	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3044_s_33	10591686	Tyrosine phosphorylation of p125FAK in platelets stimulated with a mixture of epinephrine and anti-LIBS6 antibody 30  or in platelets adherent either to fibrinogen or to immobilized immunoglobulin IgG 31 32  is blocked when PKC activity was inhibited with a specific PKC inhibitor, bisindolylmaleimide GF 109203X, suggesting that p125FAK is activated downstream of PKC. PKC-induced serine phosphorylation of p125FAK has been suggested to regulate the intracellular stability of focal adhesion kinase in mouse 3T3 cells.	transcription
57519	2	335411	7	NULL	NULL	0	NULL	anti-LIBS6 antibody 30			stimulate					p125FAK		phosphorylation of	tyrosine		NULL	platelets	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3044_s_33	10591686	Tyrosine phosphorylation of p125FAK in platelets stimulated with a mixture of epinephrine and anti-LIBS6 antibody 30  or in platelets adherent either to fibrinogen or to immobilized immunoglobulin IgG 31 32  is blocked when PKC activity was inhibited with a specific PKC inhibitor, bisindolylmaleimide GF 109203X, suggesting that p125FAK is activated downstream of PKC. PKC-induced serine phosphorylation of p125FAK has been suggested to regulate the intracellular stability of focal adhesion kinase in mouse 3T3 cells.	transcription
57520	3	335411	7	NULL	NULL	0	NULL	statement 1			occur simulataneous with					statement 2					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3044_s_33	10591686	Tyrosine phosphorylation of p125FAK in platelets stimulated with a mixture of epinephrine and anti-LIBS6 antibody 30  or in platelets adherent either to fibrinogen or to immobilized immunoglobulin IgG 31 32  is blocked when PKC activity was inhibited with a specific PKC inhibitor, bisindolylmaleimide GF 109203X, suggesting that p125FAK is activated downstream of PKC. PKC-induced serine phosphorylation of p125FAK has been suggested to regulate the intracellular stability of focal adhesion kinase in mouse 3T3 cells.	transcription
57521	4	335411	7	NULL	NULL	0	NULL	fibrinogen		platelets adherent  to	stimulate					p125FAK		phosphorylation of	tyrosine		NULL	platelets	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3044_s_33	10591686	Tyrosine phosphorylation of p125FAK in platelets stimulated with a mixture of epinephrine and anti-LIBS6 antibody 30  or in platelets adherent either to fibrinogen or to immobilized immunoglobulin IgG 31 32  is blocked when PKC activity was inhibited with a specific PKC inhibitor, bisindolylmaleimide GF 109203X, suggesting that p125FAK is activated downstream of PKC. PKC-induced serine phosphorylation of p125FAK has been suggested to regulate the intracellular stability of focal adhesion kinase in mouse 3T3 cells.	transcription
57522	5	335411	7	NULL	NULL	0	NULL	IgG		platelets adherent  to immobilized	stimulate					p125FAK		phosphorylation of	tyrosine		NULL	platelets	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3044_s_33	10591686	Tyrosine phosphorylation of p125FAK in platelets stimulated with a mixture of epinephrine and anti-LIBS6 antibody 30  or in platelets adherent either to fibrinogen or to immobilized immunoglobulin IgG 31 32  is blocked when PKC activity was inhibited with a specific PKC inhibitor, bisindolylmaleimide GF 109203X, suggesting that p125FAK is activated downstream of PKC. PKC-induced serine phosphorylation of p125FAK has been suggested to regulate the intracellular stability of focal adhesion kinase in mouse 3T3 cells.	transcription
57523	6	335411	7	NULL	NULL	0	NULL	statement 3			is an alternative to					statement 4					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3044_s_33	10591686	Tyrosine phosphorylation of p125FAK in platelets stimulated with a mixture of epinephrine and anti-LIBS6 antibody 30  or in platelets adherent either to fibrinogen or to immobilized immunoglobulin IgG 31 32  is blocked when PKC activity was inhibited with a specific PKC inhibitor, bisindolylmaleimide GF 109203X, suggesting that p125FAK is activated downstream of PKC. PKC-induced serine phosphorylation of p125FAK has been suggested to regulate the intracellular stability of focal adhesion kinase in mouse 3T3 cells.	transcription
57524	7	335411	7	NULL	NULL	0	NULL	bisindolylmaleimide			inhibits					PKC		activity of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3044_s_33	10591686	Tyrosine phosphorylation of p125FAK in platelets stimulated with a mixture of epinephrine and anti-LIBS6 antibody 30  or in platelets adherent either to fibrinogen or to immobilized immunoglobulin IgG 31 32  is blocked when PKC activity was inhibited with a specific PKC inhibitor, bisindolylmaleimide GF 109203X, suggesting that p125FAK is activated downstream of PKC. PKC-induced serine phosphorylation of p125FAK has been suggested to regulate the intracellular stability of focal adhesion kinase in mouse 3T3 cells.	transcription
57525	8	335411	7	NULL	NULL	0	NULL	GF 109203X			inhibits					PKC		activity of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3044_s_33	10591686	Tyrosine phosphorylation of p125FAK in platelets stimulated with a mixture of epinephrine and anti-LIBS6 antibody 30  or in platelets adherent either to fibrinogen or to immobilized immunoglobulin IgG 31 32  is blocked when PKC activity was inhibited with a specific PKC inhibitor, bisindolylmaleimide GF 109203X, suggesting that p125FAK is activated downstream of PKC. PKC-induced serine phosphorylation of p125FAK has been suggested to regulate the intracellular stability of focal adhesion kinase in mouse 3T3 cells.	transcription
57526	9	335411	7	NULL	NULL	0	NULL	statement 3			is an alternative to					statement 5					NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3044_s_33	10591686	Tyrosine phosphorylation of p125FAK in platelets stimulated with a mixture of epinephrine and anti-LIBS6 antibody 30  or in platelets adherent either to fibrinogen or to immobilized immunoglobulin IgG 31 32  is blocked when PKC activity was inhibited with a specific PKC inhibitor, bisindolylmaleimide GF 109203X, suggesting that p125FAK is activated downstream of PKC. PKC-induced serine phosphorylation of p125FAK has been suggested to regulate the intracellular stability of focal adhesion kinase in mouse 3T3 cells.	transcription
57527	10	335411	7	NULL	NULL	0	NULL	statement 4			is an alternative to					statement 5					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3044_s_33	10591686	Tyrosine phosphorylation of p125FAK in platelets stimulated with a mixture of epinephrine and anti-LIBS6 antibody 30  or in platelets adherent either to fibrinogen or to immobilized immunoglobulin IgG 31 32  is blocked when PKC activity was inhibited with a specific PKC inhibitor, bisindolylmaleimide GF 109203X, suggesting that p125FAK is activated downstream of PKC. PKC-induced serine phosphorylation of p125FAK has been suggested to regulate the intracellular stability of focal adhesion kinase in mouse 3T3 cells.	transcription
57528	11	335411	7	NULL	NULL	0	NULL	statement 7			blocks					statement 3					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3044_s_33	10591686	Tyrosine phosphorylation of p125FAK in platelets stimulated with a mixture of epinephrine and anti-LIBS6 antibody 30  or in platelets adherent either to fibrinogen or to immobilized immunoglobulin IgG 31 32  is blocked when PKC activity was inhibited with a specific PKC inhibitor, bisindolylmaleimide GF 109203X, suggesting that p125FAK is activated downstream of PKC. PKC-induced serine phosphorylation of p125FAK has been suggested to regulate the intracellular stability of focal adhesion kinase in mouse 3T3 cells.	transcription
57529	12	335411	7	NULL	NULL	0	NULL	statement 7			blocks					statement 4					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3044_s_33	10591686	Tyrosine phosphorylation of p125FAK in platelets stimulated with a mixture of epinephrine and anti-LIBS6 antibody 30  or in platelets adherent either to fibrinogen or to immobilized immunoglobulin IgG 31 32  is blocked when PKC activity was inhibited with a specific PKC inhibitor, bisindolylmaleimide GF 109203X, suggesting that p125FAK is activated downstream of PKC. PKC-induced serine phosphorylation of p125FAK has been suggested to regulate the intracellular stability of focal adhesion kinase in mouse 3T3 cells.	transcription
57530	13	335411	7	NULL	NULL	0	NULL	statement 7			blocks					statement 5					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3044_s_33	10591686	Tyrosine phosphorylation of p125FAK in platelets stimulated with a mixture of epinephrine and anti-LIBS6 antibody 30  or in platelets adherent either to fibrinogen or to immobilized immunoglobulin IgG 31 32  is blocked when PKC activity was inhibited with a specific PKC inhibitor, bisindolylmaleimide GF 109203X, suggesting that p125FAK is activated downstream of PKC. PKC-induced serine phosphorylation of p125FAK has been suggested to regulate the intracellular stability of focal adhesion kinase in mouse 3T3 cells.	transcription
57531	14	335411	7	NULL	NULL	0	NULL	statement 8			blocks					statement 3					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3044_s_33	10591686	Tyrosine phosphorylation of p125FAK in platelets stimulated with a mixture of epinephrine and anti-LIBS6 antibody 30  or in platelets adherent either to fibrinogen or to immobilized immunoglobulin IgG 31 32  is blocked when PKC activity was inhibited with a specific PKC inhibitor, bisindolylmaleimide GF 109203X, suggesting that p125FAK is activated downstream of PKC. PKC-induced serine phosphorylation of p125FAK has been suggested to regulate the intracellular stability of focal adhesion kinase in mouse 3T3 cells.	transcription
57532	15	335411	7	NULL	NULL	0	NULL	statement 8			blocks					statement 4					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3044_s_33	10591686	Tyrosine phosphorylation of p125FAK in platelets stimulated with a mixture of epinephrine and anti-LIBS6 antibody 30  or in platelets adherent either to fibrinogen or to immobilized immunoglobulin IgG 31 32  is blocked when PKC activity was inhibited with a specific PKC inhibitor, bisindolylmaleimide GF 109203X, suggesting that p125FAK is activated downstream of PKC. PKC-induced serine phosphorylation of p125FAK has been suggested to regulate the intracellular stability of focal adhesion kinase in mouse 3T3 cells.	transcription
57533	16	335411	7	NULL	NULL	0	NULL	statement 8			blocks					statement 5					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3044_s_33	10591686	Tyrosine phosphorylation of p125FAK in platelets stimulated with a mixture of epinephrine and anti-LIBS6 antibody 30  or in platelets adherent either to fibrinogen or to immobilized immunoglobulin IgG 31 32  is blocked when PKC activity was inhibited with a specific PKC inhibitor, bisindolylmaleimide GF 109203X, suggesting that p125FAK is activated downstream of PKC. PKC-induced serine phosphorylation of p125FAK has been suggested to regulate the intracellular stability of focal adhesion kinase in mouse 3T3 cells.	transcription
57534	17	335411	7	NULL	NULL	0	NULL	bisindolylmaleimide			is a type of					PKC inhibitor					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3044_s_33	10591686	Tyrosine phosphorylation of p125FAK in platelets stimulated with a mixture of epinephrine and anti-LIBS6 antibody 30  or in platelets adherent either to fibrinogen or to immobilized immunoglobulin IgG 31 32  is blocked when PKC activity was inhibited with a specific PKC inhibitor, bisindolylmaleimide GF 109203X, suggesting that p125FAK is activated downstream of PKC. PKC-induced serine phosphorylation of p125FAK has been suggested to regulate the intracellular stability of focal adhesion kinase in mouse 3T3 cells.	transcription
57535	18	335411	7	NULL	NULL	0	NULL	GF 109203X			is a type of					PKC inhibitor					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3044_s_33	10591686	Tyrosine phosphorylation of p125FAK in platelets stimulated with a mixture of epinephrine and anti-LIBS6 antibody 30  or in platelets adherent either to fibrinogen or to immobilized immunoglobulin IgG 31 32  is blocked when PKC activity was inhibited with a specific PKC inhibitor, bisindolylmaleimide GF 109203X, suggesting that p125FAK is activated downstream of PKC. PKC-induced serine phosphorylation of p125FAK has been suggested to regulate the intracellular stability of focal adhesion kinase in mouse 3T3 cells.	transcription
57536	19	335411	7	NULL	NULL	0	NULL	p125FAK			activated					PKC		downstream of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3044_s_33	10591686	Tyrosine phosphorylation of p125FAK in platelets stimulated with a mixture of epinephrine and anti-LIBS6 antibody 30  or in platelets adherent either to fibrinogen or to immobilized immunoglobulin IgG 31 32  is blocked when PKC activity was inhibited with a specific PKC inhibitor, bisindolylmaleimide GF 109203X, suggesting that p125FAK is activated downstream of PKC. PKC-induced serine phosphorylation of p125FAK has been suggested to regulate the intracellular stability of focal adhesion kinase in mouse 3T3 cells.	transcription
57537	20	335411	7	NULL	NULL	0	NULL	PKC			induce					p125FAK		phosphorylation of	serine		NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3044_s_33	10591686	Tyrosine phosphorylation of p125FAK in platelets stimulated with a mixture of epinephrine and anti-LIBS6 antibody 30  or in platelets adherent either to fibrinogen or to immobilized immunoglobulin IgG 31 32  is blocked when PKC activity was inhibited with a specific PKC inhibitor, bisindolylmaleimide GF 109203X, suggesting that p125FAK is activated downstream of PKC. PKC-induced serine phosphorylation of p125FAK has been suggested to regulate the intracellular stability of focal adhesion kinase in mouse 3T3 cells.	transcription
57538	21	335411	7	NULL	NULL	0	NULL	statement 20			regulate					 focal adhesion kinase		intracellular stability of 			NULL	mouse 3T3 cells	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3044_s_33	10591686	Tyrosine phosphorylation of p125FAK in platelets stimulated with a mixture of epinephrine and anti-LIBS6 antibody 30  or in platelets adherent either to fibrinogen or to immobilized immunoglobulin IgG 31 32  is blocked when PKC activity was inhibited with a specific PKC inhibitor, bisindolylmaleimide GF 109203X, suggesting that p125FAK is activated downstream of PKC. PKC-induced serine phosphorylation of p125FAK has been suggested to regulate the intracellular stability of focal adhesion kinase in mouse 3T3 cells.	transcription
57539	22	335411	7	NULL	NULL	0	NULL	statement 11			suggest					statement 19					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3044_s_33	10591686	Tyrosine phosphorylation of p125FAK in platelets stimulated with a mixture of epinephrine and anti-LIBS6 antibody 30  or in platelets adherent either to fibrinogen or to immobilized immunoglobulin IgG 31 32  is blocked when PKC activity was inhibited with a specific PKC inhibitor, bisindolylmaleimide GF 109203X, suggesting that p125FAK is activated downstream of PKC. PKC-induced serine phosphorylation of p125FAK has been suggested to regulate the intracellular stability of focal adhesion kinase in mouse 3T3 cells.	transcription
57540	23	335411	7	NULL	NULL	0	NULL	statement 12			suggest					statement 19					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3044_s_33	10591686	Tyrosine phosphorylation of p125FAK in platelets stimulated with a mixture of epinephrine and anti-LIBS6 antibody 30  or in platelets adherent either to fibrinogen or to immobilized immunoglobulin IgG 31 32  is blocked when PKC activity was inhibited with a specific PKC inhibitor, bisindolylmaleimide GF 109203X, suggesting that p125FAK is activated downstream of PKC. PKC-induced serine phosphorylation of p125FAK has been suggested to regulate the intracellular stability of focal adhesion kinase in mouse 3T3 cells.	transcription
57541	24	335411	7	NULL	NULL	0	NULL	statement 13			suggest					statement 19					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3044_s_33	10591686	Tyrosine phosphorylation of p125FAK in platelets stimulated with a mixture of epinephrine and anti-LIBS6 antibody 30  or in platelets adherent either to fibrinogen or to immobilized immunoglobulin IgG 31 32  is blocked when PKC activity was inhibited with a specific PKC inhibitor, bisindolylmaleimide GF 109203X, suggesting that p125FAK is activated downstream of PKC. PKC-induced serine phosphorylation of p125FAK has been suggested to regulate the intracellular stability of focal adhesion kinase in mouse 3T3 cells.	transcription
57542	25	335411	7	NULL	NULL	0	NULL	statement 14			suggest					statement 19					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3044_s_33	10591686	Tyrosine phosphorylation of p125FAK in platelets stimulated with a mixture of epinephrine and anti-LIBS6 antibody 30  or in platelets adherent either to fibrinogen or to immobilized immunoglobulin IgG 31 32  is blocked when PKC activity was inhibited with a specific PKC inhibitor, bisindolylmaleimide GF 109203X, suggesting that p125FAK is activated downstream of PKC. PKC-induced serine phosphorylation of p125FAK has been suggested to regulate the intracellular stability of focal adhesion kinase in mouse 3T3 cells.	transcription
57543	26	335411	7	NULL	NULL	0	NULL	statement 15			suggest					statement 19					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3044_s_33	10591686	Tyrosine phosphorylation of p125FAK in platelets stimulated with a mixture of epinephrine and anti-LIBS6 antibody 30  or in platelets adherent either to fibrinogen or to immobilized immunoglobulin IgG 31 32  is blocked when PKC activity was inhibited with a specific PKC inhibitor, bisindolylmaleimide GF 109203X, suggesting that p125FAK is activated downstream of PKC. PKC-induced serine phosphorylation of p125FAK has been suggested to regulate the intracellular stability of focal adhesion kinase in mouse 3T3 cells.	transcription
57544	27	335411	7	NULL	NULL	0	NULL	statement 16			suggest					statement 19					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_12_3044_s_33	10591686	Tyrosine phosphorylation of p125FAK in platelets stimulated with a mixture of epinephrine and anti-LIBS6 antibody 30  or in platelets adherent either to fibrinogen or to immobilized immunoglobulin IgG 31 32  is blocked when PKC activity was inhibited with a specific PKC inhibitor, bisindolylmaleimide GF 109203X, suggesting that p125FAK is activated downstream of PKC. PKC-induced serine phosphorylation of p125FAK has been suggested to regulate the intracellular stability of focal adhesion kinase in mouse 3T3 cells.	transcription
57545	1	335412	7	NULL	NULL	0	NULL	L-DOPA			induce					melanin		excess production of			NULL	 highly melanized organisms 	NULL	NULL	NULL	NULL	gw70_eukaryotcell_5_6_916_s_189	16757739	To address this, we exposed native melanized  Pneumocystis (basal amounts of melanins) and highly melanized organisms (excessive melanin production induced by L-DOPA) to either UV irradiation or desiccation.	transcription
78767	1	335413	6	NULL	NULL	0	NULL	riboflavin	GP		bind					DOPA-melanin	GP				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_282_3_1228_s_732	9316830	Studies on equilibrium binding of riboflavin to DOPA-melanin and some spectroscopic characteristics of flavin-melanin complex.	transcription
57546	1	335413	7	NULL	NULL	0	NULL	riboflavin 			bind					DOPA-melanin 					NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_282_3_1228_s_732	9316830	Studies on equilibrium binding of riboflavin to DOPA-melanin and some spectroscopic characteristics of flavin-melanin complex.	transcription
78768	1	335414	6	NULL	NULL	0	NULL	DDC	GP		is					dopa decarboxylase	GP				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_10_591_s_20	10837223	Thus, dopa decarboxylase (DDC) catalyzes the conversion of dopa to dopamine, which is a precursor for both melanin and papiliochrome synthesis (  Figure 1c).	transcription
78769	2	335414	6	NULL	NULL	0	NULL	dopa	Chemical		is converted to					dopamine	Chemical				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_10_591_s_20	10837223	Thus, dopa decarboxylase (DDC) catalyzes the conversion of dopa to dopamine, which is a precursor for both melanin and papiliochrome synthesis (  Figure 1c).	transcription
78770	3	335414	6	NULL	NULL	0	NULL	DDC	GP		catalyzes					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_10_591_s_20	10837223	Thus, dopa decarboxylase (DDC) catalyzes the conversion of dopa to dopamine, which is a precursor for both melanin and papiliochrome synthesis (  Figure 1c).	transcription
78771	4	335414	6	NULL	NULL	0	NULL	dopamine	Chemical		is a precursor for					melanin 	Chemical	synthesis of 			NULL		0	NULL	NULL	NULL	gw60_currbiol_10_10_591_s_20	10837223	Thus, dopa decarboxylase (DDC) catalyzes the conversion of dopa to dopamine, which is a precursor for both melanin and papiliochrome synthesis (  Figure 1c).	transcription
78772	5	335414	6	NULL	NULL	0	NULL	dopamine	Chemical		is a precursor for					papiliochrome	Chemical	synthesis of 			NULL		0	NULL	NULL	NULL	gw60_currbiol_10_10_591_s_20	10837223	Thus, dopa decarboxylase (DDC) catalyzes the conversion of dopa to dopamine, which is a precursor for both melanin and papiliochrome synthesis (  Figure 1c).	transcription
57547	1	335414	7	NULL	NULL	0	NULL	dopa			converted to					dopamine					NULL		0	NULL	NULL	NULL	gw60_currbiol_10_10_591_s_20	10837223	Thus, dopa decarboxylase (DDC) catalyzes the conversion of dopa to dopamine, which is a precursor for both melanin and papiliochrome synthesis (  Figure 1c).	transcription
57548	2	335414	7	NULL	NULL	0	NULL	DDC			catalyze					statement 1					NULL		0	NULL	NULL	NULL	gw60_currbiol_10_10_591_s_20	10837223	Thus, dopa decarboxylase (DDC) catalyzes the conversion of dopa to dopamine, which is a precursor for both melanin and papiliochrome synthesis (  Figure 1c).	transcription
57549	3	335414	7	NULL	NULL	0	NULL	statement 1			is a precursor of					melanin		biosynthesis of			NULL		0	NULL	NULL	NULL	gw60_currbiol_10_10_591_s_20	10837223	Thus, dopa decarboxylase (DDC) catalyzes the conversion of dopa to dopamine, which is a precursor for both melanin and papiliochrome synthesis (  Figure 1c).	transcription
57550	4	335414	7	NULL	NULL	0	NULL	statement 1			is a precursor of					papiliochrome		biosynthesis of			NULL		0	NULL	NULL	NULL	gw60_currbiol_10_10_591_s_20	10837223	Thus, dopa decarboxylase (DDC) catalyzes the conversion of dopa to dopamine, which is a precursor for both melanin and papiliochrome synthesis (  Figure 1c).	transcription
57551	5	335414	7	NULL	NULL	0	NULL	DDC			is					dopa decarboxylase					NULL		0	NULL	NULL	NULL	gw60_currbiol_10_10_591_s_20	10837223	Thus, dopa decarboxylase (DDC) catalyzes the conversion of dopa to dopamine, which is a precursor for both melanin and papiliochrome synthesis (  Figure 1c).	transcription
57552	1	335415	7	NULL	NULL	0	NULL	melanin		cell wall of melanized yeast cells 	reacts with					L-dopa Abs		C. neoformans melanin			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-immunol_160_12_9637518_s_7	9637518	Furthermore, the  experiments demonstrate 1) a sensitive ELISA for the measurement of Ab  to melanin, 2) that mice mount an intense Ab response to fungal melanin  that includes Abs of IgM and IgG isotypes, 3) that melanins from different  sources have cross-reactive epitopes, and 4) melanin in the cell wall  of melanized yeast cells reacts with Abs raised to L-dopa C. neoformans  melanin.	transcription
57553	2	335415	7	NULL	NULL	0	NULL	melanin		fungal	mounts					IgM antibody					NULL	mice	0	NULL	NULL	NULL	abs-batch0720-0739_j-immunol_160_12_9637518_s_7	9637518	Furthermore, the  experiments demonstrate 1) a sensitive ELISA for the measurement of Ab  to melanin, 2) that mice mount an intense Ab response to fungal melanin  that includes Abs of IgM and IgG isotypes, 3) that melanins from different  sources have cross-reactive epitopes, and 4) melanin in the cell wall  of melanized yeast cells reacts with Abs raised to L-dopa C. neoformans  melanin.	transcription
57554	3	335415	7	NULL	NULL	0	NULL	melanin		fungal	mounts					IgG antibody					NULL	mice	NULL	NULL	NULL	NULL	abs-batch0720-0739_j-immunol_160_12_9637518_s_7	9637518	Furthermore, the  experiments demonstrate 1) a sensitive ELISA for the measurement of Ab  to melanin, 2) that mice mount an intense Ab response to fungal melanin  that includes Abs of IgM and IgG isotypes, 3) that melanins from different  sources have cross-reactive epitopes, and 4) melanin in the cell wall  of melanized yeast cells reacts with Abs raised to L-dopa C. neoformans  melanin.	transcription
78780	1	335416	6	NULL	NULL	0	NULL	glyphosate	Chemical		inhibits					phenoloxidase activity	Process	Pneumocystis			NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_5_6_916_s_144	16757739	Panel D shows that glyphosate inhibition of  Pneumocystis phenoloxidase activity impairs the L-DOPA-driven generation of  Pneumocystis melanin pigment.	transcription
78781	2	335416	6	NULL	NULL	0	NULL	L-DOPA	Chemical		drives					melanin pigment	Chemical	generation of;; Pneumocystis			NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_5_6_916_s_144	16757739	Panel D shows that glyphosate inhibition of  Pneumocystis phenoloxidase activity impairs the L-DOPA-driven generation of  Pneumocystis melanin pigment.	transcription
78782	3	335416	6	NULL	NULL	0	NULL	statement 1	Process		impairs					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_5_6_916_s_144	16757739	Panel D shows that glyphosate inhibition of  Pneumocystis phenoloxidase activity impairs the L-DOPA-driven generation of  Pneumocystis melanin pigment.	transcription
57555	1	335416	7	NULL	NULL	0	NULL	glyphosate			inhibits					Pneumocystis phenoloxidase		activity of			NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_5_6_916_s_144	16757739	Panel D shows that glyphosate inhibition of  Pneumocystis phenoloxidase activity impairs the L-DOPA-driven generation of  Pneumocystis melanin pigment.	transcription
57556	2	335416	7	NULL	NULL	0	NULL	L-DOPA			drives					Pneumocystis melanin pigment		generation of			NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_5_6_916_s_144	16757739	Panel D shows that glyphosate inhibition of  Pneumocystis phenoloxidase activity impairs the L-DOPA-driven generation of  Pneumocystis melanin pigment.	transcription
57557	3	335416	7	NULL	NULL	0	NULL	statement 1			impairs					statement 2					NULL		0	NULL	NULL	NULL	gw70_eukaryotcell_5_6_916_s_144	16757739	Panel D shows that glyphosate inhibition of  Pneumocystis phenoloxidase activity impairs the L-DOPA-driven generation of  Pneumocystis melanin pigment.	transcription
78783	1	335417	6	NULL	NULL	0	NULL	tyrosine	GP		is converted to					DOPA	Chemical				NULL		0	NULL	NULL	NULL	gw70_pnas_103_2_353_s_28	16384915	Tyr catalyzes the conversion of tyrosine to DOPA, which is an essential and rate-limiting step in melanin synthesis.	transcription
78784	2	335417	6	NULL	NULL	0	NULL	Tyr	GP		catalyzes					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_103_2_353_s_28	16384915	Tyr catalyzes the conversion of tyrosine to DOPA, which is an essential and rate-limiting step in melanin synthesis.	transcription
78785	3	335417	6	NULL	NULL	0	NULL	statement 1	Process		plays a role in					melanin 	Chemical	synthesis of 			NULL		0	NULL	NULL	NULL	gw70_pnas_103_2_353_s_28	16384915	Tyr catalyzes the conversion of tyrosine to DOPA, which is an essential and rate-limiting step in melanin synthesis.	transcription
57558	1	335417	7	NULL	NULL	0	NULL	 tyrosine			converted to					DOPA					NULL		0	NULL	NULL	NULL	gw70_pnas_103_2_353_s_28	16384915	Tyr catalyzes the conversion of tyrosine to DOPA, which is an essential and rate-limiting step in melanin synthesis.	transcription
57559	2	335417	7	NULL	NULL	0	NULL	Tyr			catalyze					statement 1					NULL		0	NULL	NULL	NULL	gw70_pnas_103_2_353_s_28	16384915	Tyr catalyzes the conversion of tyrosine to DOPA, which is an essential and rate-limiting step in melanin synthesis.	transcription
57560	3	335417	7	NULL	NULL	0	NULL	statement 1			rate limiting step in					melanin		synthesis of			NULL		0	NULL	NULL	NULL	gw70_pnas_103_2_353_s_28	16384915	Tyr catalyzes the conversion of tyrosine to DOPA, which is an essential and rate-limiting step in melanin synthesis.	transcription
57561	1	335418	7	NULL	NULL	0	NULL	melanin			synthesized from					L-DOPA					NULL	cytoplasmic yeast extract	0	NULL	NULL	NULL	gw60_infectimmun_69_9_5760_s_8	11500453	Nonreducing polyacrylamide gel electrophoresis of cytoplasmic yeast extract revealed a protein that catalyzed melanin synthesis from L-DOPA.	transcription
78786	1	335419	6	NULL	NULL	0	NULL	melanin-binding peptides	GP		inhibits					C. neoformans	Organism	growth of 			NULL		0	NULL	NULL	NULL	gw70_microbesinfect_7_4_789_s_53	15823515	The growth of  C. neoformans was also inhibited by melanin-binding peptides   [13] and glyphosate   [14], which inhibited autopolymerization of  l-dopa and oxidation of  l-epinephrine by cryptococcal cells.	transcription
78787	2	335419	6	NULL	NULL	0	NULL	glyphosate	Chemical		inhibits					C. neoformans	Organism	growth of 			NULL		0	NULL	NULL	NULL	gw70_microbesinfect_7_4_789_s_53	15823515	The growth of  C. neoformans was also inhibited by melanin-binding peptides   [13] and glyphosate   [14], which inhibited autopolymerization of  l-dopa and oxidation of  l-epinephrine by cryptococcal cells.	transcription
78788	3	335419	6	NULL	NULL	NULL	NULL	cryptococcal cells	Cell		autopolymerizes					l-dopa	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_microbesinfect_7_4_789_s_53	15823515	The growth of  C. neoformans was also inhibited by melanin-binding peptides   [13] and glyphosate   [14], which inhibited autopolymerization of  l-dopa and oxidation of  l-epinephrine by cryptococcal cells.	transcription
78789	4	335419	6	NULL	NULL	0	NULL	cryptococcal cells	Cell		autopolymerizes					l-epinephrine	Chemical				NULL		0	NULL	NULL	NULL	gw70_microbesinfect_7_4_789_s_53	15823515	The growth of  C. neoformans was also inhibited by melanin-binding peptides   [13] and glyphosate   [14], which inhibited autopolymerization of  l-dopa and oxidation of  l-epinephrine by cryptococcal cells.	transcription
78790	5	335419	6	NULL	NULL	0	NULL	statement 1	Process		inhibits					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_microbesinfect_7_4_789_s_53	15823515	The growth of  C. neoformans was also inhibited by melanin-binding peptides   [13] and glyphosate   [14], which inhibited autopolymerization of  l-dopa and oxidation of  l-epinephrine by cryptococcal cells.	transcription
78791	6	335419	6	NULL	NULL	0	NULL	statement 1	Process		inhibits					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_microbesinfect_7_4_789_s_53	15823515	The growth of  C. neoformans was also inhibited by melanin-binding peptides   [13] and glyphosate   [14], which inhibited autopolymerization of  l-dopa and oxidation of  l-epinephrine by cryptococcal cells.	transcription
78792	7	335419	6	NULL	NULL	0	NULL	statement 2	Process		inhibits					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_microbesinfect_7_4_789_s_53	15823515	The growth of  C. neoformans was also inhibited by melanin-binding peptides   [13] and glyphosate   [14], which inhibited autopolymerization of  l-dopa and oxidation of  l-epinephrine by cryptococcal cells.	transcription
78793	8	335419	6	NULL	NULL	0	NULL	statement 2	Process		inhibits					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_microbesinfect_7_4_789_s_53	15823515	The growth of  C. neoformans was also inhibited by melanin-binding peptides   [13] and glyphosate   [14], which inhibited autopolymerization of  l-dopa and oxidation of  l-epinephrine by cryptococcal cells.	transcription
57562	1	335419	7	NULL	NULL	0	NULL	 melanin-binding peptides			inhibits					C. neoformans		growth of			NULL		0	NULL	NULL	NULL	gw70_microbesinfect_7_4_789_s_53	15823515	The growth of  C. neoformans was also inhibited by melanin-binding peptides   [13] and glyphosate   [14], which inhibited autopolymerization of  l-dopa and oxidation of  l-epinephrine by cryptococcal cells.	transcription
57563	2	335419	7	NULL	NULL	0	NULL	glyphosate			inhibits					C. neoformans		growth of			NULL		0	NULL	NULL	NULL	gw70_microbesinfect_7_4_789_s_53	15823515	The growth of  C. neoformans was also inhibited by melanin-binding peptides   [13] and glyphosate   [14], which inhibited autopolymerization of  l-dopa and oxidation of  l-epinephrine by cryptococcal cells.	transcription
57564	3	335419	7	NULL	NULL	0	NULL	 l-dopa			undergoes					autopolymerization					NULL		0	NULL	NULL	NULL	gw70_microbesinfect_7_4_789_s_53	15823515	The growth of  C. neoformans was also inhibited by melanin-binding peptides   [13] and glyphosate   [14], which inhibited autopolymerization of  l-dopa and oxidation of  l-epinephrine by cryptococcal cells.	transcription
57565	4	335419	7	NULL	NULL	0	NULL	cryptococcal cells			oxidize					l-epinephrine					NULL		0	NULL	NULL	NULL	gw70_microbesinfect_7_4_789_s_53	15823515	The growth of  C. neoformans was also inhibited by melanin-binding peptides   [13] and glyphosate   [14], which inhibited autopolymerization of  l-dopa and oxidation of  l-epinephrine by cryptococcal cells.	transcription
57566	5	335419	7	NULL	NULL	0	NULL	melanin-binding peptides			inhibits					statement 3					NULL		NULL	NULL	NULL	NULL	gw70_microbesinfect_7_4_789_s_53	15823515	The growth of  C. neoformans was also inhibited by melanin-binding peptides   [13] and glyphosate   [14], which inhibited autopolymerization of  l-dopa and oxidation of  l-epinephrine by cryptococcal cells.	transcription
57567	6	335419	7	NULL	NULL	0	NULL	melanin-binding peptides			inhibits					statement 4					NULL		NULL	NULL	NULL	NULL	gw70_microbesinfect_7_4_789_s_53	15823515	The growth of  C. neoformans was also inhibited by melanin-binding peptides   [13] and glyphosate   [14], which inhibited autopolymerization of  l-dopa and oxidation of  l-epinephrine by cryptococcal cells.	transcription
57568	7	335419	7	NULL	NULL	0	NULL	glyphosate 			inhibits					statement 3					NULL		NULL	NULL	NULL	NULL	gw70_microbesinfect_7_4_789_s_53	15823515	The growth of  C. neoformans was also inhibited by melanin-binding peptides   [13] and glyphosate   [14], which inhibited autopolymerization of  l-dopa and oxidation of  l-epinephrine by cryptococcal cells.	transcription
57569	8	335419	7	NULL	NULL	0	NULL	glyphosate 			inhibits					statement 4					NULL		0	NULL	NULL	NULL	gw70_microbesinfect_7_4_789_s_53	15823515	The growth of  C. neoformans was also inhibited by melanin-binding peptides   [13] and glyphosate   [14], which inhibited autopolymerization of  l-dopa and oxidation of  l-epinephrine by cryptococcal cells.	transcription
78794	1	335420	6	NULL	NULL	0	NULL	MelC2	GP		forms					DOPA melanin	Chemical				NULL	Streptomyces	0	NULL	NULL	NULL	gw70_jbacteriol_187_23_8149_s_15	16291687	The representative of the tyrosinases responsible for the formation of DOPA melanin in  Streptomyces is MelC2 ( ), which is a copper-containing monooxygenase that catalyzes the  o-hydroxylation of monophenols and the oxidation of  o-diphenols to yield  o-quinones using molecular oxygen ( ).	transcription
78795	2	335420	6	NULL	NULL	0	NULL	MelC2	Chemical		is a type of					copper-containing monooxygenase 					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_23_8149_s_15	16291687	The representative of the tyrosinases responsible for the formation of DOPA melanin in  Streptomyces is MelC2 ( ), which is a copper-containing monooxygenase that catalyzes the  o-hydroxylation of monophenols and the oxidation of  o-diphenols to yield  o-quinones using molecular oxygen ( ).	transcription
78796	3	335420	6	NULL	NULL	0	NULL	MelC2	GP		catalyzes					monophenols	Chemical	o-hydroxylation of 			NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_23_8149_s_15	16291687	The representative of the tyrosinases responsible for the formation of DOPA melanin in  Streptomyces is MelC2 ( ), which is a copper-containing monooxygenase that catalyzes the  o-hydroxylation of monophenols and the oxidation of  o-diphenols to yield  o-quinones using molecular oxygen ( ).	transcription
78797	4	335420	6	NULL	NULL	0	NULL	o-diphenol	Chemical		is oxidized to					o-quinone	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_23_8149_s_15	16291687	The representative of the tyrosinases responsible for the formation of DOPA melanin in  Streptomyces is MelC2 ( ), which is a copper-containing monooxygenase that catalyzes the  o-hydroxylation of monophenols and the oxidation of  o-diphenols to yield  o-quinones using molecular oxygen ( ).	transcription
57570	1	335420	7	NULL	NULL	0	NULL	MelC2 			responsible for					DOPA melanin		formation of			NULL	Streptomyces	NULL	NULL	NULL	NULL	gw70_jbacteriol_187_23_8149_s_15	16291687	The representative of the tyrosinases responsible for the formation of DOPA melanin in  Streptomyces is MelC2 ( ), which is a copper-containing monooxygenase that catalyzes the  o-hydroxylation of monophenols and the oxidation of  o-diphenols to yield  o-quinones using molecular oxygen ( ).	transcription
57571	2	335420	7	NULL	NULL	0	NULL	MelC2			is a type of					tyrosinases					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_23_8149_s_15	16291687	The representative of the tyrosinases responsible for the formation of DOPA melanin in  Streptomyces is MelC2 ( ), which is a copper-containing monooxygenase that catalyzes the  o-hydroxylation of monophenols and the oxidation of  o-diphenols to yield  o-quinones using molecular oxygen ( ).	transcription
57572	3	335420	7	NULL	NULL	0	NULL	MelC2 			is a type of					copper-containing monooxygenase					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_23_8149_s_15	16291687	The representative of the tyrosinases responsible for the formation of DOPA melanin in  Streptomyces is MelC2 ( ), which is a copper-containing monooxygenase that catalyzes the  o-hydroxylation of monophenols and the oxidation of  o-diphenols to yield  o-quinones using molecular oxygen ( ).	transcription
57573	4	335420	7	NULL	NULL	0	NULL	monophenols		o-hydroxylation of	yield					o-quinones					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_23_8149_s_15	16291687	The representative of the tyrosinases responsible for the formation of DOPA melanin in  Streptomyces is MelC2 ( ), which is a copper-containing monooxygenase that catalyzes the  o-hydroxylation of monophenols and the oxidation of  o-diphenols to yield  o-quinones using molecular oxygen ( ).	transcription
57574	5	335420	7	NULL	NULL	0	NULL	o-diphenols 		oxidation of	yield					o-quinones					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_23_8149_s_15	16291687	The representative of the tyrosinases responsible for the formation of DOPA melanin in  Streptomyces is MelC2 ( ), which is a copper-containing monooxygenase that catalyzes the  o-hydroxylation of monophenols and the oxidation of  o-diphenols to yield  o-quinones using molecular oxygen ( ).	transcription
57575	6	335420	7	NULL	NULL	0	NULL	statement 4			involves					molecular oxygen					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_23_8149_s_15	16291687	The representative of the tyrosinases responsible for the formation of DOPA melanin in  Streptomyces is MelC2 ( ), which is a copper-containing monooxygenase that catalyzes the  o-hydroxylation of monophenols and the oxidation of  o-diphenols to yield  o-quinones using molecular oxygen ( ).	transcription
57576	7	335420	7	NULL	NULL	0	NULL	statement 5			involves					molecular oxygen					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_23_8149_s_15	16291687	The representative of the tyrosinases responsible for the formation of DOPA melanin in  Streptomyces is MelC2 ( ), which is a copper-containing monooxygenase that catalyzes the  o-hydroxylation of monophenols and the oxidation of  o-diphenols to yield  o-quinones using molecular oxygen ( ).	transcription
78798	1	335421	6	NULL	NULL	0	NULL	BrY	GP		excretes					HGA	Chemical				NULL	S. algae	0	NULL	NULL	NULL	gw60_applenvironmicrob_68_5_2436_s_218	11976119	In addition previous work demonstrated that HGA, but not DOPA, is excreted by  S. algae BrY and melanin production by  S. algae BrY is inhibited by sulcotrione, a specific inhibitor of the enzyme  p-hydroxyphenylpyruvate dioxygenase, which produces HGA ( 39).	transcription
78799	2	335421	6	NULL	NULL	0	NULL	BrY	GP		produces					melanin	Chemical				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_5_2436_s_218	11976119	In addition previous work demonstrated that HGA, but not DOPA, is excreted by  S. algae BrY and melanin production by  S. algae BrY is inhibited by sulcotrione, a specific inhibitor of the enzyme  p-hydroxyphenylpyruvate dioxygenase, which produces HGA ( 39).	transcription
78800	3	335421	6	NULL	NULL	0	NULL	sulcotrione	Chemical		inhibits					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_5_2436_s_218	11976119	In addition previous work demonstrated that HGA, but not DOPA, is excreted by  S. algae BrY and melanin production by  S. algae BrY is inhibited by sulcotrione, a specific inhibitor of the enzyme  p-hydroxyphenylpyruvate dioxygenase, which produces HGA ( 39).	transcription
78801	4	335421	6	NULL	NULL	0	NULL	sulcotrione	Chemical		is an					p-hydroxyphenylpyruvate dioxygenase	GP	inhibitor of 			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_5_2436_s_218	11976119	In addition previous work demonstrated that HGA, but not DOPA, is excreted by  S. algae BrY and melanin production by  S. algae BrY is inhibited by sulcotrione, a specific inhibitor of the enzyme  p-hydroxyphenylpyruvate dioxygenase, which produces HGA ( 39).	transcription
78802	5	335421	6	NULL	NULL	0	NULL	p-hydroxyphenylpyruvate dioxygenase	GP		produces					HGA	Chemical				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_5_2436_s_218	11976119	In addition previous work demonstrated that HGA, but not DOPA, is excreted by  S. algae BrY and melanin production by  S. algae BrY is inhibited by sulcotrione, a specific inhibitor of the enzyme  p-hydroxyphenylpyruvate dioxygenase, which produces HGA ( 39).	transcription
57577	1	335421	7	NULL	NULL	0	NULL	HGA			is excreted by					BrY		S. algae			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_5_2436_s_218	11976119	In addition previous work demonstrated that HGA, but not DOPA, is excreted by  S. algae BrY and melanin production by  S. algae BrY is inhibited by sulcotrione, a specific inhibitor of the enzyme  p-hydroxyphenylpyruvate dioxygenase, which produces HGA ( 39).	transcription
57578	2	335421	7	NULL	NULL	0	NULL	BrY		 S. algae 	produce					melanin					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_5_2436_s_218	11976119	In addition previous work demonstrated that HGA, but not DOPA, is excreted by  S. algae BrY and melanin production by  S. algae BrY is inhibited by sulcotrione, a specific inhibitor of the enzyme  p-hydroxyphenylpyruvate dioxygenase, which produces HGA ( 39).	transcription
57579	3	335421	7	NULL	NULL	0	NULL	sulcotrione			inhibit					statement 2					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_5_2436_s_218	11976119	In addition previous work demonstrated that HGA, but not DOPA, is excreted by  S. algae BrY and melanin production by  S. algae BrY is inhibited by sulcotrione, a specific inhibitor of the enzyme  p-hydroxyphenylpyruvate dioxygenase, which produces HGA ( 39).	transcription
57580	4	335421	7	NULL	NULL	0	NULL	p-hydroxyphenylpyruvate dioxygenase			produce					HGA					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_5_2436_s_218	11976119	In addition previous work demonstrated that HGA, but not DOPA, is excreted by  S. algae BrY and melanin production by  S. algae BrY is inhibited by sulcotrione, a specific inhibitor of the enzyme  p-hydroxyphenylpyruvate dioxygenase, which produces HGA ( 39).	transcription
57581	5	335421	7	NULL	NULL	0	NULL	sulcotrione			inhibitor of		specific			 p-hydroxyphenylpyruvate dioxygenase					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_5_2436_s_218	11976119	In addition previous work demonstrated that HGA, but not DOPA, is excreted by  S. algae BrY and melanin production by  S. algae BrY is inhibited by sulcotrione, a specific inhibitor of the enzyme  p-hydroxyphenylpyruvate dioxygenase, which produces HGA ( 39).	transcription
57582	6	335421	7	NULL	NULL	0	NULL	DOPA			is not excreted by					BrY		S. algae			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_68_5_2436_s_218	11976119	In addition previous work demonstrated that HGA, but not DOPA, is excreted by  S. algae BrY and melanin production by  S. algae BrY is inhibited by sulcotrione, a specific inhibitor of the enzyme  p-hydroxyphenylpyruvate dioxygenase, which produces HGA ( 39).	transcription
78803	1	335422	6	NULL	NULL	0	NULL	dopa	Chemical		regulates					retinal mitosis	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_18_23_9948_s_255	9822750	Ilia M, Jeffery G (1998) Retinal mitosis is regulated by dopa, a melanin precursor that may influence the time at which cells exit the cell cycle: analysis of patterns of cell production in pigmented and albino retinae.	transcription
78804	2	335422	6	NULL	NULL	0	NULL	dopa	Chemical		is a precursor for					melanin 	Chemical				NULL		0	NULL	NULL	NULL	gw60_jneurosci_18_23_9948_s_255	9822750	Ilia M, Jeffery G (1998) Retinal mitosis is regulated by dopa, a melanin precursor that may influence the time at which cells exit the cell cycle: analysis of patterns of cell production in pigmented and albino retinae.	transcription
57583	1	335422	7	NULL	NULL	0	NULL	Retinal mitosis			is regulated by					dopa					NULL		0	NULL	NULL	NULL	gw60_jneurosci_18_23_9948_s_255	9822750	Ilia M, Jeffery G (1998) Retinal mitosis is regulated by dopa, a melanin precursor that may influence the time at which cells exit the cell cycle: analysis of patterns of cell production in pigmented and albino retinae.	transcription
57584	2	335422	7	NULL	NULL	0	NULL	dopa			is a precursor of					melanin					NULL		0	NULL	NULL	NULL	gw60_jneurosci_18_23_9948_s_255	9822750	Ilia M, Jeffery G (1998) Retinal mitosis is regulated by dopa, a melanin precursor that may influence the time at which cells exit the cell cycle: analysis of patterns of cell production in pigmented and albino retinae.	transcription
57585	3	335422	7	NULL	NULL	0	NULL	dopa			influence					cell cycle		time at which cells exit 			NULL		0	NULL	NULL	NULL	gw60_jneurosci_18_23_9948_s_255	9822750	Ilia M, Jeffery G (1998) Retinal mitosis is regulated by dopa, a melanin precursor that may influence the time at which cells exit the cell cycle: analysis of patterns of cell production in pigmented and albino retinae.	transcription
57586	1	335423	7	NULL	NULL	0	NULL	L-dopa			added to					Cryptococcus					NULL		0	NULL	NULL	NULL	gw60_infectimmun_67_11_6034_s_5	10531264	Addition of L-dopa to  Cryptococcus to produce melanin in a laccase-positive strain resulted in a slight increase in protection of  C. neoformans from the antifungal activity of macrophages ([25.4  plus-or-minus  3.4]% versus [28.9  plus-or-minus  1.2]% killing).	transcription
57587	2	335423	7	NULL	NULL	0	NULL	statement 1			produce					melanin					NULL	laccase-positive strain	0	NULL	NULL	NULL	gw60_infectimmun_67_11_6034_s_5	10531264	Addition of L-dopa to  Cryptococcus to produce melanin in a laccase-positive strain resulted in a slight increase in protection of  C. neoformans from the antifungal activity of macrophages ([25.4  plus-or-minus  3.4]% versus [28.9  plus-or-minus  1.2]% killing).	transcription
57588	4	335423	7	NULL	NULL	0	NULL	statement 2			increase					statement 3					NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_67_11_6034_s_5	10531264	Addition of L-dopa to  Cryptococcus to produce melanin in a laccase-positive strain resulted in a slight increase in protection of  C. neoformans from the antifungal activity of macrophages ([25.4  plus-or-minus  3.4]% versus [28.9  plus-or-minus  1.2]% killing).	transcription
57589	3	335423	7	NULL	NULL	0	NULL	C. neoformans			protected from					macrophages		antifungal activity of			NULL		0	NULL	NULL	NULL	gw60_infectimmun_67_11_6034_s_5	10531264	Addition of L-dopa to  Cryptococcus to produce melanin in a laccase-positive strain resulted in a slight increase in protection of  C. neoformans from the antifungal activity of macrophages ([25.4  plus-or-minus  3.4]% versus [28.9  plus-or-minus  1.2]% killing).	transcription
78805	1	335424	6	NULL	NULL	0	NULL	NB-DNJ	Chemical		is					N-butyldeoxynojirimycin	Chemical				NULL		0	NULL	NULL	NULL	gw60_cellbiol_155_3_369_s_65	11673476	Indeed, treatment of MEB4 cells with  N-butyldeoxynojirimycin (NB-DNJ), a potent inhibitor of the ER alpha-glucosidases and of maturation of tyrosinase into the active conformation ( Petrescu et al., 1997), completely inhibited melanin formation unless exogenous L-DOPA was added to bypass the requirement for tyrosinase ( Fig. 2 B).	transcription
78806	2	335424	6	NULL	NULL	0	NULL	NB-DNJ	Chemical		inhibits					ER alpha-glucosidases	Chemical				NULL		0	NULL	NULL	NULL	gw60_cellbiol_155_3_369_s_65	11673476	Indeed, treatment of MEB4 cells with  N-butyldeoxynojirimycin (NB-DNJ), a potent inhibitor of the ER alpha-glucosidases and of maturation of tyrosinase into the active conformation ( Petrescu et al., 1997), completely inhibited melanin formation unless exogenous L-DOPA was added to bypass the requirement for tyrosinase ( Fig. 2 B).	transcription
57590	1	335424	7	NULL	NULL	0	NULL	NB-DNJ			inhibitor of		potent			ER alpha-glucosidases					NULL		0	NULL	NULL	NULL	gw60_cellbiol_155_3_369_s_65	11673476	Indeed, treatment of MEB4 cells with  N-butyldeoxynojirimycin (NB-DNJ), a potent inhibitor of the ER alpha-glucosidases and of maturation of tyrosinase into the active conformation ( Petrescu et al., 1997), completely inhibited melanin formation unless exogenous L-DOPA was added to bypass the requirement for tyrosinase ( Fig. 2 B).	transcription
57591	2	335424	7	NULL	NULL	0	NULL	tyrosinase			matures to					active conformation					NULL		0	NULL	NULL	NULL	gw60_cellbiol_155_3_369_s_65	11673476	Indeed, treatment of MEB4 cells with  N-butyldeoxynojirimycin (NB-DNJ), a potent inhibitor of the ER alpha-glucosidases and of maturation of tyrosinase into the active conformation ( Petrescu et al., 1997), completely inhibited melanin formation unless exogenous L-DOPA was added to bypass the requirement for tyrosinase ( Fig. 2 B).	transcription
57592	3	335424	7	NULL	NULL	0	NULL	NB-DNJ			inhibits		completely			melanin		formation of			NULL	MEB4 cells	NULL	NULL	NULL	NULL	gw60_cellbiol_155_3_369_s_65	11673476	Indeed, treatment of MEB4 cells with  N-butyldeoxynojirimycin (NB-DNJ), a potent inhibitor of the ER alpha-glucosidases and of maturation of tyrosinase into the active conformation ( Petrescu et al., 1997), completely inhibited melanin formation unless exogenous L-DOPA was added to bypass the requirement for tyrosinase ( Fig. 2 B).	transcription
57593	4	335424	7	NULL	NULL	0	NULL	statement 2			inhibits		completely			melanin		formation of			NULL	MEB4 cells	NULL	NULL	NULL	NULL	gw60_cellbiol_155_3_369_s_65	11673476	Indeed, treatment of MEB4 cells with  N-butyldeoxynojirimycin (NB-DNJ), a potent inhibitor of the ER alpha-glucosidases and of maturation of tyrosinase into the active conformation ( Petrescu et al., 1997), completely inhibited melanin formation unless exogenous L-DOPA was added to bypass the requirement for tyrosinase ( Fig. 2 B).	transcription
57594	5	335424	7	NULL	NULL	0	NULL	L-DOPA		exogenous	reverse					statement 3					NULL		0	NULL	NULL	NULL	gw60_cellbiol_155_3_369_s_65	11673476	Indeed, treatment of MEB4 cells with  N-butyldeoxynojirimycin (NB-DNJ), a potent inhibitor of the ER alpha-glucosidases and of maturation of tyrosinase into the active conformation ( Petrescu et al., 1997), completely inhibited melanin formation unless exogenous L-DOPA was added to bypass the requirement for tyrosinase ( Fig. 2 B).	transcription
57595	6	335424	7	NULL	NULL	0	NULL	L-DOPA		exogenous	reverse					statement 4					NULL		0	NULL	NULL	NULL	gw60_cellbiol_155_3_369_s_65	11673476	Indeed, treatment of MEB4 cells with  N-butyldeoxynojirimycin (NB-DNJ), a potent inhibitor of the ER alpha-glucosidases and of maturation of tyrosinase into the active conformation ( Petrescu et al., 1997), completely inhibited melanin formation unless exogenous L-DOPA was added to bypass the requirement for tyrosinase ( Fig. 2 B).	transcription
57596	7	335424	7	NULL	NULL	0	NULL	L-DOPA		addition of	bypass 					tyrosinase		requirement for			NULL		0	NULL	NULL	NULL	gw60_cellbiol_155_3_369_s_65	11673476	Indeed, treatment of MEB4 cells with  N-butyldeoxynojirimycin (NB-DNJ), a potent inhibitor of the ER alpha-glucosidases and of maturation of tyrosinase into the active conformation ( Petrescu et al., 1997), completely inhibited melanin formation unless exogenous L-DOPA was added to bypass the requirement for tyrosinase ( Fig. 2 B).	transcription
57597	8	335424	7	NULL	NULL	0	NULL	NB-DNJ			is					N-butyldeoxynojirimycin					NULL		0	NULL	NULL	NULL	gw60_cellbiol_155_3_369_s_65	11673476	Indeed, treatment of MEB4 cells with  N-butyldeoxynojirimycin (NB-DNJ), a potent inhibitor of the ER alpha-glucosidases and of maturation of tyrosinase into the active conformation ( Petrescu et al., 1997), completely inhibited melanin formation unless exogenous L-DOPA was added to bypass the requirement for tyrosinase ( Fig. 2 B).	transcription
78807	1	335425	6	NULL	NULL	0	NULL	melanin	Chemical		is produced by					C. neoformans	Organism				NULL		0	NULL	NULL	NULL	gw60_infectimmun_67_11_6034_s_97	10531264	While melanin produced by  C. neoformans in the presence of L-dopa inhibited phagocytosis by AMs ([10.0  plus-or-minus  2.0]% with the laccase-positive strain versus [19.4  plus-or-minus  0.4]% with the laccase-deficient strain), the phagocytosis indices of the two strains were similar in the absence of L-dopa substrate ([17.0  plus-or-minus  1.0]% versus [18.2  plus-or-minus  1.3]%) (Fig.  2).	transcription
78808	2	335425	6	NULL	NULL	0	NULL	statement 1	Process		occurs in presence of					L-dopa	Chemical				NULL		0	NULL	NULL	NULL	gw60_infectimmun_67_11_6034_s_97	10531264	While melanin produced by  C. neoformans in the presence of L-dopa inhibited phagocytosis by AMs ([10.0  plus-or-minus  2.0]% with the laccase-positive strain versus [19.4  plus-or-minus  0.4]% with the laccase-deficient strain), the phagocytosis indices of the two strains were similar in the absence of L-dopa substrate ([17.0  plus-or-minus  1.0]% versus [18.2  plus-or-minus  1.3]%) (Fig.  2).	transcription
78809	3	335425	6	NULL	NULL	0	NULL	AM	CellComponent		plays a role in					phagocytosis	Process				NULL		0	NULL	NULL	NULL	gw60_infectimmun_67_11_6034_s_97	10531264	While melanin produced by  C. neoformans in the presence of L-dopa inhibited phagocytosis by AMs ([10.0  plus-or-minus  2.0]% with the laccase-positive strain versus [19.4  plus-or-minus  0.4]% with the laccase-deficient strain), the phagocytosis indices of the two strains were similar in the absence of L-dopa substrate ([17.0  plus-or-minus  1.0]% versus [18.2  plus-or-minus  1.3]%) (Fig.  2).	transcription
78810	4	335425	6	NULL	NULL	0	NULL	statement 1	Process		inhibits					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_infectimmun_67_11_6034_s_97	10531264	While melanin produced by  C. neoformans in the presence of L-dopa inhibited phagocytosis by AMs ([10.0  plus-or-minus  2.0]% with the laccase-positive strain versus [19.4  plus-or-minus  0.4]% with the laccase-deficient strain), the phagocytosis indices of the two strains were similar in the absence of L-dopa substrate ([17.0  plus-or-minus  1.0]% versus [18.2  plus-or-minus  1.3]%) (Fig.  2).	transcription
57599	1	335425	7	NULL	NULL	0	NULL	C. neoformans			produce					melanin					NULL		0	NULL	NULL	NULL	gw60_infectimmun_67_11_6034_s_97	10531264	While melanin produced by  C. neoformans in the presence of L-dopa inhibited phagocytosis by AMs ([10.0  plus-or-minus  2.0]% with the laccase-positive strain versus [19.4  plus-or-minus  0.4]% with the laccase-deficient strain), the phagocytosis indices of the two strains were similar in the absence of L-dopa substrate ([17.0  plus-or-minus  1.0]% versus [18.2  plus-or-minus  1.3]%) (Fig.  2).	transcription
57600	2	335425	7	NULL	NULL	0	NULL	statement 1			in the presence of					L-dopa					NULL		0	NULL	NULL	NULL	gw60_infectimmun_67_11_6034_s_97	10531264	While melanin produced by  C. neoformans in the presence of L-dopa inhibited phagocytosis by AMs ([10.0  plus-or-minus  2.0]% with the laccase-positive strain versus [19.4  plus-or-minus  0.4]% with the laccase-deficient strain), the phagocytosis indices of the two strains were similar in the absence of L-dopa substrate ([17.0  plus-or-minus  1.0]% versus [18.2  plus-or-minus  1.3]%) (Fig.  2).	transcription
57621	3	335425	7	NULL	NULL	0	NULL	melanin			inhibits					AMs		phagocytosis by			NULL		0	NULL	NULL	NULL	gw60_infectimmun_67_11_6034_s_97	10531264	While melanin produced by  C. neoformans in the presence of L-dopa inhibited phagocytosis by AMs ([10.0  plus-or-minus  2.0]% with the laccase-positive strain versus [19.4  plus-or-minus  0.4]% with the laccase-deficient strain), the phagocytosis indices of the two strains were similar in the absence of L-dopa substrate ([17.0  plus-or-minus  1.0]% versus [18.2  plus-or-minus  1.3]%) (Fig.  2).	transcription
78811	1	335426	6	NULL	NULL	0	NULL	trimethyllysine	AminoAcid		is an intermediate for					L-carnitine	AminoAcid	biosynthesis of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_39_36262_s_298	12089149	In contrast, trimethyllysine and lysine, an intermediate and a precursor of L-carnitine biosynthesis, respectively, had no apparent inhibitory effect on CT2-mediated carnitine uptake.	transcription
78812	2	335426	6	NULL	NULL	0	NULL	lysine	AminoAcid		is a precursor for					L-carnitine	AminoAcid	biosynthesis of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_39_36262_s_298	12089149	In contrast, trimethyllysine and lysine, an intermediate and a precursor of L-carnitine biosynthesis, respectively, had no apparent inhibitory effect on CT2-mediated carnitine uptake.	transcription
57622	1	335426	7	NULL	NULL	0	NULL	 trimethyllysine			intermediate of					L-carnitine		biosynthesis of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_39_36262_s_298	12089149	In contrast, trimethyllysine and lysine, an intermediate and a precursor of L-carnitine biosynthesis, respectively, had no apparent inhibitory effect on CT2-mediated carnitine uptake.	transcription
57623	2	335426	7	NULL	NULL	0	NULL	lysine			precursor of					L-carnitine		biosynthesis of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_39_36262_s_298	12089149	In contrast, trimethyllysine and lysine, an intermediate and a precursor of L-carnitine biosynthesis, respectively, had no apparent inhibitory effect on CT2-mediated carnitine uptake.	transcription
57624	3	335426	7	NULL	NULL	0	NULL	CT2			mediates					carnitine		uptake of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_39_36262_s_298	12089149	In contrast, trimethyllysine and lysine, an intermediate and a precursor of L-carnitine biosynthesis, respectively, had no apparent inhibitory effect on CT2-mediated carnitine uptake.	transcription
57625	4	335426	7	NULL	NULL	0	NULL	statement 1			has no inhibitory effect on					statement 3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_39_36262_s_298	12089149	In contrast, trimethyllysine and lysine, an intermediate and a precursor of L-carnitine biosynthesis, respectively, had no apparent inhibitory effect on CT2-mediated carnitine uptake.	transcription
57626	5	335426	7	NULL	NULL	0	NULL	statement 2			has no inhibitory effect on					statement 3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_39_36262_s_298	12089149	In contrast, trimethyllysine and lysine, an intermediate and a precursor of L-carnitine biosynthesis, respectively, had no apparent inhibitory effect on CT2-mediated carnitine uptake.	transcription
78813	1	335427	6	NULL	NULL	0	NULL	lysine	AminoAcid		did not affect					L-carnitine	AminoAcid	uptake of 			NULL		0	NULL	NULL	NULL	gw60_embo_18_21_5843_s_179	10545096	Amino acids including lysine, serine, leucine and threonine did not affect the uptake of L-carnitine.	transcription
78814	2	335427	6	NULL	NULL	0	NULL	serine	AminoAcid		did not affect					L-carnitine	AminoAcid	uptake of 			NULL		0	NULL	NULL	NULL	gw60_embo_18_21_5843_s_179	10545096	Amino acids including lysine, serine, leucine and threonine did not affect the uptake of L-carnitine.	transcription
78815	3	335427	6	NULL	NULL	0	NULL	leucine	AminoAcid		did not affect					L-carnitine	AminoAcid	uptake of 			NULL		0	NULL	NULL	NULL	gw60_embo_18_21_5843_s_179	10545096	Amino acids including lysine, serine, leucine and threonine did not affect the uptake of L-carnitine.	transcription
78816	4	335427	6	NULL	NULL	0	NULL	threonine	AminoAcid		did not affect					L-carnitine	AminoAcid	uptake of 			NULL		0	NULL	NULL	NULL	gw60_embo_18_21_5843_s_179	10545096	Amino acids including lysine, serine, leucine and threonine did not affect the uptake of L-carnitine.	transcription
57627	1	335427	7	NULL	NULL	0	NULL	lysine			does not affect					L-carnitine		uptake of			NULL		0	NULL	NULL	NULL	gw60_embo_18_21_5843_s_179	10545096	Amino acids including lysine, serine, leucine and threonine did not affect the uptake of L-carnitine.	transcription
57628	2	335427	7	NULL	NULL	0	NULL	serine			does not affect					L-carnitine		uptake of			NULL		0	NULL	NULL	NULL	gw60_embo_18_21_5843_s_179	10545096	Amino acids including lysine, serine, leucine and threonine did not affect the uptake of L-carnitine.	transcription
57629	3	335427	7	NULL	NULL	0	NULL	leucine			does not affect					L-carnitine		uptake of			NULL		0	NULL	NULL	NULL	gw60_embo_18_21_5843_s_179	10545096	Amino acids including lysine, serine, leucine and threonine did not affect the uptake of L-carnitine.	transcription
57630	4	335427	7	NULL	NULL	0	NULL	threonine			does not affect					L-carnitine		uptake of			NULL		0	NULL	NULL	NULL	gw60_embo_18_21_5843_s_179	10545096	Amino acids including lysine, serine, leucine and threonine did not affect the uptake of L-carnitine.	transcription
57631	5	335427	7	NULL	NULL	0	NULL	lysine			is a type of					amino acid					NULL		0	NULL	NULL	NULL	gw60_embo_18_21_5843_s_179	10545096	Amino acids including lysine, serine, leucine and threonine did not affect the uptake of L-carnitine.	transcription
57632	6	335427	7	NULL	NULL	0	NULL	serine			is a type of					amino acid					NULL		0	NULL	NULL	NULL	gw60_embo_18_21_5843_s_179	10545096	Amino acids including lysine, serine, leucine and threonine did not affect the uptake of L-carnitine.	transcription
57633	7	335427	7	NULL	NULL	0	NULL	leucine			is a type of					amino acid					NULL		0	NULL	NULL	NULL	gw60_embo_18_21_5843_s_179	10545096	Amino acids including lysine, serine, leucine and threonine did not affect the uptake of L-carnitine.	transcription
57634	8	335427	7	NULL	NULL	0	NULL	threonine			is a type of					amino acid					NULL		0	NULL	NULL	NULL	gw60_embo_18_21_5843_s_179	10545096	Amino acids including lysine, serine, leucine and threonine did not affect the uptake of L-carnitine.	transcription
57635	1	335428	7	NULL	NULL	0	NULL	gamma-butyrobetaine			inhibit					carnitine transport activity		free			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_289_1_93_s_229	10086992	As examples of inhibition of free carnitine transport activity by carnitine analogs, gamma-butyrobetaine, acetylcarnitine, and lysine are known to function as inhibitors (Huth and Shug, 1980  ; Bahl et al., 1981  ).	transcription
57636	2	335428	7	NULL	NULL	0	NULL	acetylcarnitine			inhibit					carnitine transport activity		free			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_289_1_93_s_229	10086992	As examples of inhibition of free carnitine transport activity by carnitine analogs, gamma-butyrobetaine, acetylcarnitine, and lysine are known to function as inhibitors (Huth and Shug, 1980  ; Bahl et al., 1981  ).	transcription
57637	3	335428	7	NULL	NULL	0	NULL	lysine			inhibit					carnitine transport activity		free			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_289_1_93_s_229	10086992	As examples of inhibition of free carnitine transport activity by carnitine analogs, gamma-butyrobetaine, acetylcarnitine, and lysine are known to function as inhibitors (Huth and Shug, 1980  ; Bahl et al., 1981  ).	transcription
57638	4	335428	7	NULL	NULL	0	NULL	gamma-butyrobetaine			is a type of					carnitine analog					NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_289_1_93_s_229	10086992	As examples of inhibition of free carnitine transport activity by carnitine analogs, gamma-butyrobetaine, acetylcarnitine, and lysine are known to function as inhibitors (Huth and Shug, 1980  ; Bahl et al., 1981  ).	transcription
57639	5	335428	7	NULL	NULL	0	NULL	acetylcarnitine			is a type of					carnitine analog					NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_289_1_93_s_229	10086992	As examples of inhibition of free carnitine transport activity by carnitine analogs, gamma-butyrobetaine, acetylcarnitine, and lysine are known to function as inhibitors (Huth and Shug, 1980  ; Bahl et al., 1981  ).	transcription
57640	6	335428	7	NULL	NULL	0	NULL	 lysine			is a type of					carnitine transport activity		free			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_289_1_93_s_229	10086992	As examples of inhibition of free carnitine transport activity by carnitine analogs, gamma-butyrobetaine, acetylcarnitine, and lysine are known to function as inhibitors (Huth and Shug, 1980  ; Bahl et al., 1981  ).	transcription
78817	1	335429	6	NULL	NULL	0	NULL	lysine	AminoAcid		is converted to					Carnitine	AminoAcid				NULL		0	NULL	NULL	NULL	gw70_pnas_103_7_2434_s_41	16467150	ALDH9 is a key enzyme in converting lysine to carnitine ( ), which provides substrates for the carnitine shuttle system mediated by CPT1 and Slc25a20, whereas peroxisomal enoyl-CoA isomerase and hydratase play important roles in peroxisomal fatty acid beta-oxidation.	transcription
78818	2	335429	6	NULL	NULL	0	NULL	ALDH9	GP		catalyzes					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_103_7_2434_s_41	16467150	ALDH9 is a key enzyme in converting lysine to carnitine ( ), which provides substrates for the carnitine shuttle system mediated by CPT1 and Slc25a20, whereas peroxisomal enoyl-CoA isomerase and hydratase play important roles in peroxisomal fatty acid beta-oxidation.	transcription
78819	3	335429	6	NULL	NULL	0	NULL	peroxisomal enoyl-CoA isomerase	GP		plays a role in					fatty acid beta-oxidation	Process	peroxisomal			NULL		0	NULL	NULL	NULL	gw70_pnas_103_7_2434_s_41	16467150	ALDH9 is a key enzyme in converting lysine to carnitine ( ), which provides substrates for the carnitine shuttle system mediated by CPT1 and Slc25a20, whereas peroxisomal enoyl-CoA isomerase and hydratase play important roles in peroxisomal fatty acid beta-oxidation.	transcription
78820	4	335429	6	NULL	NULL	0	NULL	peroxisomal enoyl-CoA hydratase	GP		plays a role in					peroxisomal fatty acid beta-oxidation	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_103_7_2434_s_41	16467150	ALDH9 is a key enzyme in converting lysine to carnitine ( ), which provides substrates for the carnitine shuttle system mediated by CPT1 and Slc25a20, whereas peroxisomal enoyl-CoA isomerase and hydratase play important roles in peroxisomal fatty acid beta-oxidation.	transcription
57641	1	335429	7	NULL	NULL	0	NULL	lysine			converted to					carnitine					NULL		0	NULL	NULL	NULL	gw70_pnas_103_7_2434_s_41	16467150	ALDH9 is a key enzyme in converting lysine to carnitine ( ), which provides substrates for the carnitine shuttle system mediated by CPT1 and Slc25a20, whereas peroxisomal enoyl-CoA isomerase and hydratase play important roles in peroxisomal fatty acid beta-oxidation.	transcription
57642	2	335429	7	NULL	NULL	0	NULL	ALDH9			carries out					statement 1					NULL		0	NULL	NULL	NULL	gw70_pnas_103_7_2434_s_41	16467150	ALDH9 is a key enzyme in converting lysine to carnitine ( ), which provides substrates for the carnitine shuttle system mediated by CPT1 and Slc25a20, whereas peroxisomal enoyl-CoA isomerase and hydratase play important roles in peroxisomal fatty acid beta-oxidation.	transcription
57643	3	335429	7	NULL	NULL	0	NULL	carinitine			substrate for					 carnitine shuttle system					NULL		0	NULL	NULL	NULL	gw70_pnas_103_7_2434_s_41	16467150	ALDH9 is a key enzyme in converting lysine to carnitine ( ), which provides substrates for the carnitine shuttle system mediated by CPT1 and Slc25a20, whereas peroxisomal enoyl-CoA isomerase and hydratase play important roles in peroxisomal fatty acid beta-oxidation.	transcription
57644	4	335429	7	NULL	NULL	0	NULL	CPT1			mediates					statement 3					NULL		0	NULL	NULL	NULL	gw70_pnas_103_7_2434_s_41	16467150	ALDH9 is a key enzyme in converting lysine to carnitine ( ), which provides substrates for the carnitine shuttle system mediated by CPT1 and Slc25a20, whereas peroxisomal enoyl-CoA isomerase and hydratase play important roles in peroxisomal fatty acid beta-oxidation.	transcription
57645	5	335429	7	NULL	NULL	0	NULL	Slc25a20			mediates					statement 3					NULL		0	NULL	NULL	NULL	gw70_pnas_103_7_2434_s_41	16467150	ALDH9 is a key enzyme in converting lysine to carnitine ( ), which provides substrates for the carnitine shuttle system mediated by CPT1 and Slc25a20, whereas peroxisomal enoyl-CoA isomerase and hydratase play important roles in peroxisomal fatty acid beta-oxidation.	transcription
57646	6	335429	7	NULL	NULL	0	NULL	peroxisomal enoyl-CoA isomerase			play important role in					fatty acid beta-oxidation		peroxisomal			NULL		0	NULL	NULL	NULL	gw70_pnas_103_7_2434_s_41	16467150	ALDH9 is a key enzyme in converting lysine to carnitine ( ), which provides substrates for the carnitine shuttle system mediated by CPT1 and Slc25a20, whereas peroxisomal enoyl-CoA isomerase and hydratase play important roles in peroxisomal fatty acid beta-oxidation.	transcription
57647	7	335429	7	NULL	NULL	0	NULL	hydratase			play important role in					fatty acid beta-oxidation		peroxisomal			NULL		0	NULL	NULL	NULL	gw70_pnas_103_7_2434_s_41	16467150	ALDH9 is a key enzyme in converting lysine to carnitine ( ), which provides substrates for the carnitine shuttle system mediated by CPT1 and Slc25a20, whereas peroxisomal enoyl-CoA isomerase and hydratase play important roles in peroxisomal fatty acid beta-oxidation.	transcription
57648	1	335430	7	NULL	NULL	0	NULL	OCTN2		rat	mediates					carnitine transport					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_51_40064_s_229	11010964	Strong inhibitory effects were observed with carnitine-related compounds, including acylcarnitines and gamma-butyrobetaine, whereas lysine, gamma-aminobutyrate, or choline showed negligible or weak inhibitory effect; these are consistent with observations in human and rat OCTN2-mediated carnitine transport ( 9,  23,  42).	transcription
57649	2	335430	7	NULL	NULL	0	NULL	OCTN2		human	mediates					carnitine transport					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_51_40064_s_229	11010964	Strong inhibitory effects were observed with carnitine-related compounds, including acylcarnitines and gamma-butyrobetaine, whereas lysine, gamma-aminobutyrate, or choline showed negligible or weak inhibitory effect; these are consistent with observations in human and rat OCTN2-mediated carnitine transport ( 9,  23,  42).	transcription
57650	3	335430	7	NULL	NULL	0	NULL	acylcarnitines			shows					strong inhibitory effect					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_51_40064_s_229	11010964	Strong inhibitory effects were observed with carnitine-related compounds, including acylcarnitines and gamma-butyrobetaine, whereas lysine, gamma-aminobutyrate, or choline showed negligible or weak inhibitory effect; these are consistent with observations in human and rat OCTN2-mediated carnitine transport ( 9,  23,  42).	transcription
57651	4	335430	7	NULL	NULL	0	NULL	gamma-butyrobetaine			shows					strong inhibitory effect					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_51_40064_s_229	11010964	Strong inhibitory effects were observed with carnitine-related compounds, including acylcarnitines and gamma-butyrobetaine, whereas lysine, gamma-aminobutyrate, or choline showed negligible or weak inhibitory effect; these are consistent with observations in human and rat OCTN2-mediated carnitine transport ( 9,  23,  42).	transcription
57652	5	335430	7	NULL	NULL	0	NULL	lysine			shows					weak inhibitory effect					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_51_40064_s_229	11010964	Strong inhibitory effects were observed with carnitine-related compounds, including acylcarnitines and gamma-butyrobetaine, whereas lysine, gamma-aminobutyrate, or choline showed negligible or weak inhibitory effect; these are consistent with observations in human and rat OCTN2-mediated carnitine transport ( 9,  23,  42).	transcription
57653	6	335430	7	NULL	NULL	0	NULL	 gamma-aminobutyrate			shows					weak inhibitory effect					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_51_40064_s_229	11010964	Strong inhibitory effects were observed with carnitine-related compounds, including acylcarnitines and gamma-butyrobetaine, whereas lysine, gamma-aminobutyrate, or choline showed negligible or weak inhibitory effect; these are consistent with observations in human and rat OCTN2-mediated carnitine transport ( 9,  23,  42).	transcription
57654	7	335430	7	NULL	NULL	0	NULL	choline			shows					weak inhibitory effect					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_51_40064_s_229	11010964	Strong inhibitory effects were observed with carnitine-related compounds, including acylcarnitines and gamma-butyrobetaine, whereas lysine, gamma-aminobutyrate, or choline showed negligible or weak inhibitory effect; these are consistent with observations in human and rat OCTN2-mediated carnitine transport ( 9,  23,  42).	transcription
57655	1	335431	7	NULL	NULL	0	NULL	Ant1p		reconstituted 	does not catalyze					phosphate		homo-exchanges of			NULL		0	NULL	NULL	NULL	gw60_embo_20_18_5049_s_154	11566870	Furthermore, reconstituted Ant1p did not catalyze the homo-exchanges of phosphate, pyruvate, malonate, succinate, malate, oxoglutarate, ketoisocaproate, citrate, carnitine, ornithine, lysine, arginine, histidine, glutathione, choline, spermine, proline and threonine (external concentration 1 mM, internal concentration 10 mM; data not shown), all being substrates for various known mitochondrial transporters.	transcription
57656	2	335431	7	NULL	NULL	0	NULL	Ant1p		reconstituted 	does not catalyze					pyruvate		homo-exchanges of			NULL		0	NULL	NULL	NULL	gw60_embo_20_18_5049_s_154	11566870	Furthermore, reconstituted Ant1p did not catalyze the homo-exchanges of phosphate, pyruvate, malonate, succinate, malate, oxoglutarate, ketoisocaproate, citrate, carnitine, ornithine, lysine, arginine, histidine, glutathione, choline, spermine, proline and threonine (external concentration 1 mM, internal concentration 10 mM; data not shown), all being substrates for various known mitochondrial transporters.	transcription
57657	3	335431	7	NULL	NULL	0	NULL	Ant1p		reconstituted 	does not catalyze					malonate		homo-exchanges of			NULL		0	NULL	NULL	NULL	gw60_embo_20_18_5049_s_154	11566870	Furthermore, reconstituted Ant1p did not catalyze the homo-exchanges of phosphate, pyruvate, malonate, succinate, malate, oxoglutarate, ketoisocaproate, citrate, carnitine, ornithine, lysine, arginine, histidine, glutathione, choline, spermine, proline and threonine (external concentration 1 mM, internal concentration 10 mM; data not shown), all being substrates for various known mitochondrial transporters.	transcription
57658	4	335431	7	NULL	NULL	0	NULL	Ant1p		reconstituted 	does not catalyze					succinate		homo-exchanges of			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_18_5049_s_154	11566870	Furthermore, reconstituted Ant1p did not catalyze the homo-exchanges of phosphate, pyruvate, malonate, succinate, malate, oxoglutarate, ketoisocaproate, citrate, carnitine, ornithine, lysine, arginine, histidine, glutathione, choline, spermine, proline and threonine (external concentration 1 mM, internal concentration 10 mM; data not shown), all being substrates for various known mitochondrial transporters.	transcription
57659	5	335431	7	NULL	NULL	0	NULL	Ant1p		reconstituted 	does not catalyze					malate		homo-exchanges of			NULL		0	NULL	NULL	NULL	gw60_embo_20_18_5049_s_154	11566870	Furthermore, reconstituted Ant1p did not catalyze the homo-exchanges of phosphate, pyruvate, malonate, succinate, malate, oxoglutarate, ketoisocaproate, citrate, carnitine, ornithine, lysine, arginine, histidine, glutathione, choline, spermine, proline and threonine (external concentration 1 mM, internal concentration 10 mM; data not shown), all being substrates for various known mitochondrial transporters.	transcription
57660	6	335431	7	NULL	NULL	0	NULL	Ant1p		reconstituted 	does not catalyze					oxoglutarate		homo-exchanges of			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_18_5049_s_154	11566870	Furthermore, reconstituted Ant1p did not catalyze the homo-exchanges of phosphate, pyruvate, malonate, succinate, malate, oxoglutarate, ketoisocaproate, citrate, carnitine, ornithine, lysine, arginine, histidine, glutathione, choline, spermine, proline and threonine (external concentration 1 mM, internal concentration 10 mM; data not shown), all being substrates for various known mitochondrial transporters.	transcription
57661	7	335431	7	NULL	NULL	0	NULL	Ant1p		reconstituted 	does not catalyze					ketoisocaproate		homo-exchanges of			NULL		0	NULL	NULL	NULL	gw60_embo_20_18_5049_s_154	11566870	Furthermore, reconstituted Ant1p did not catalyze the homo-exchanges of phosphate, pyruvate, malonate, succinate, malate, oxoglutarate, ketoisocaproate, citrate, carnitine, ornithine, lysine, arginine, histidine, glutathione, choline, spermine, proline and threonine (external concentration 1 mM, internal concentration 10 mM; data not shown), all being substrates for various known mitochondrial transporters.	transcription
57662	8	335431	7	NULL	NULL	0	NULL	Ant1p		reconstituted 	does not catalyze					citrate		homo-exchanges of			NULL		0	NULL	NULL	NULL	gw60_embo_20_18_5049_s_154	11566870	Furthermore, reconstituted Ant1p did not catalyze the homo-exchanges of phosphate, pyruvate, malonate, succinate, malate, oxoglutarate, ketoisocaproate, citrate, carnitine, ornithine, lysine, arginine, histidine, glutathione, choline, spermine, proline and threonine (external concentration 1 mM, internal concentration 10 mM; data not shown), all being substrates for various known mitochondrial transporters.	transcription
57663	9	335431	7	NULL	NULL	0	NULL	Ant1p		reconstituted 	does not catalyze					carnitine		homo-exchanges of			NULL		0	NULL	NULL	NULL	gw60_embo_20_18_5049_s_154	11566870	Furthermore, reconstituted Ant1p did not catalyze the homo-exchanges of phosphate, pyruvate, malonate, succinate, malate, oxoglutarate, ketoisocaproate, citrate, carnitine, ornithine, lysine, arginine, histidine, glutathione, choline, spermine, proline and threonine (external concentration 1 mM, internal concentration 10 mM; data not shown), all being substrates for various known mitochondrial transporters.	transcription
57664	10	335431	7	NULL	NULL	0	NULL	Ant1p		reconstituted 	does not catalyze					ornithine		homo-exchanges of			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_18_5049_s_154	11566870	Furthermore, reconstituted Ant1p did not catalyze the homo-exchanges of phosphate, pyruvate, malonate, succinate, malate, oxoglutarate, ketoisocaproate, citrate, carnitine, ornithine, lysine, arginine, histidine, glutathione, choline, spermine, proline and threonine (external concentration 1 mM, internal concentration 10 mM; data not shown), all being substrates for various known mitochondrial transporters.	transcription
57665	11	335431	7	NULL	NULL	0	NULL	Ant1p		reconstituted 	does not catalyze					lysine		homo-exchanges of			NULL		0	NULL	NULL	NULL	gw60_embo_20_18_5049_s_154	11566870	Furthermore, reconstituted Ant1p did not catalyze the homo-exchanges of phosphate, pyruvate, malonate, succinate, malate, oxoglutarate, ketoisocaproate, citrate, carnitine, ornithine, lysine, arginine, histidine, glutathione, choline, spermine, proline and threonine (external concentration 1 mM, internal concentration 10 mM; data not shown), all being substrates for various known mitochondrial transporters.	transcription
57666	12	335431	7	NULL	NULL	0	NULL	Ant1p		reconstituted 	does not catalyze					arginine		homo-exchanges of			NULL		NULL	NULL	NULL	NULL	gw60_embo_20_18_5049_s_154	11566870	Furthermore, reconstituted Ant1p did not catalyze the homo-exchanges of phosphate, pyruvate, malonate, succinate, malate, oxoglutarate, ketoisocaproate, citrate, carnitine, ornithine, lysine, arginine, histidine, glutathione, choline, spermine, proline and threonine (external concentration 1 mM, internal concentration 10 mM; data not shown), all being substrates for various known mitochondrial transporters.	transcription
57667	13	335431	7	NULL	NULL	0	NULL	Ant1p		reconstituted 	does not catalyze					histidine		homo-exchanges of			NULL		0	NULL	NULL	NULL	gw60_embo_20_18_5049_s_154	11566870	Furthermore, reconstituted Ant1p did not catalyze the homo-exchanges of phosphate, pyruvate, malonate, succinate, malate, oxoglutarate, ketoisocaproate, citrate, carnitine, ornithine, lysine, arginine, histidine, glutathione, choline, spermine, proline and threonine (external concentration 1 mM, internal concentration 10 mM; data not shown), all being substrates for various known mitochondrial transporters.	transcription
57668	14	335431	7	NULL	NULL	0	NULL	Ant1p		reconstituted 	does not catalyze					glutathione		homo-exchanges of			NULL		0	NULL	NULL	NULL	gw60_embo_20_18_5049_s_154	11566870	Furthermore, reconstituted Ant1p did not catalyze the homo-exchanges of phosphate, pyruvate, malonate, succinate, malate, oxoglutarate, ketoisocaproate, citrate, carnitine, ornithine, lysine, arginine, histidine, glutathione, choline, spermine, proline and threonine (external concentration 1 mM, internal concentration 10 mM; data not shown), all being substrates for various known mitochondrial transporters.	transcription
57669	15	335431	7	NULL	NULL	0	NULL	Ant1p		reconstituted 	does not catalyze					choline		homo-exchanges of			NULL		0	NULL	NULL	NULL	gw60_embo_20_18_5049_s_154	11566870	Furthermore, reconstituted Ant1p did not catalyze the homo-exchanges of phosphate, pyruvate, malonate, succinate, malate, oxoglutarate, ketoisocaproate, citrate, carnitine, ornithine, lysine, arginine, histidine, glutathione, choline, spermine, proline and threonine (external concentration 1 mM, internal concentration 10 mM; data not shown), all being substrates for various known mitochondrial transporters.	transcription
57670	16	335431	7	NULL	NULL	0	NULL	Ant1p		reconstituted 	does not catalyze					spermine		homo-exchanges of			NULL		0	NULL	NULL	NULL	gw60_embo_20_18_5049_s_154	11566870	Furthermore, reconstituted Ant1p did not catalyze the homo-exchanges of phosphate, pyruvate, malonate, succinate, malate, oxoglutarate, ketoisocaproate, citrate, carnitine, ornithine, lysine, arginine, histidine, glutathione, choline, spermine, proline and threonine (external concentration 1 mM, internal concentration 10 mM; data not shown), all being substrates for various known mitochondrial transporters.	transcription
57671	17	335431	7	NULL	NULL	0	NULL	Ant1p		reconstituted 	does not catalyze					proline		homo-exchanges of			NULL		0	NULL	NULL	NULL	gw60_embo_20_18_5049_s_154	11566870	Furthermore, reconstituted Ant1p did not catalyze the homo-exchanges of phosphate, pyruvate, malonate, succinate, malate, oxoglutarate, ketoisocaproate, citrate, carnitine, ornithine, lysine, arginine, histidine, glutathione, choline, spermine, proline and threonine (external concentration 1 mM, internal concentration 10 mM; data not shown), all being substrates for various known mitochondrial transporters.	transcription
57672	18	335431	7	NULL	NULL	0	NULL	Ant1p		reconstituted 	does not catalyze					threonine		homo-exchanges of			NULL		0	NULL	NULL	NULL	gw60_embo_20_18_5049_s_154	11566870	Furthermore, reconstituted Ant1p did not catalyze the homo-exchanges of phosphate, pyruvate, malonate, succinate, malate, oxoglutarate, ketoisocaproate, citrate, carnitine, ornithine, lysine, arginine, histidine, glutathione, choline, spermine, proline and threonine (external concentration 1 mM, internal concentration 10 mM; data not shown), all being substrates for various known mitochondrial transporters.	transcription
78821	1	335432	6	NULL	NULL	0	NULL	cholate	GP		did not increase					G5G8		expression of			NULL	Fxr - / - mice	0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_220	15611112	Cholate did not increase G5G8 expression in  Fxr - / -  mice, indicating that the effect of cholate on biliary cholesterol secretion is mediated by FXR.	transcription
78822	2	335432	6	NULL	NULL	0	NULL	cholate	Chemical		effects					biliary cholesterol	Chemical	secretion of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_220	15611112	Cholate did not increase G5G8 expression in  Fxr - / -  mice, indicating that the effect of cholate on biliary cholesterol secretion is mediated by FXR.	transcription
78823	3	335432	6	NULL	NULL	0	NULL	FXR	GP		mediates					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_220	15611112	Cholate did not increase G5G8 expression in  Fxr - / -  mice, indicating that the effect of cholate on biliary cholesterol secretion is mediated by FXR.	transcription
57673	1	335432	7	NULL	NULL	0	NULL	cholate 			does not increase					G5G8		expression of			NULL	Fxr - / - mice	0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_220	15611112	Cholate did not increase G5G8 expression in  Fxr - / -  mice, indicating that the effect of cholate on biliary cholesterol secretion is mediated by FXR.	transcription
57674	2	335432	7	NULL	NULL	0	NULL	FXR			mediates					biliary cholesterol		secretion of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_220	15611112	Cholate did not increase G5G8 expression in  Fxr - / -  mice, indicating that the effect of cholate on biliary cholesterol secretion is mediated by FXR.	transcription
57675	3	335432	7	NULL	NULL	0	NULL	cholate			effect					statement 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_220	15611112	Cholate did not increase G5G8 expression in  Fxr - / -  mice, indicating that the effect of cholate on biliary cholesterol secretion is mediated by FXR.	transcription
57676	4	335432	7	NULL	NULL	0	NULL	statement 1			indicate					statement 3					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_220	15611112	Cholate did not increase G5G8 expression in  Fxr - / -  mice, indicating that the effect of cholate on biliary cholesterol secretion is mediated by FXR.	transcription
57677	1	335433	7	NULL	NULL	0	NULL	taurine			induce					CYP7A1					NULL		0	NULL	NULL	NULL	abs-batch0580-0599_life-sci_77_7_15936349_s_14	15936349	The overall results suggest that there are differences between  mice and rats in susceptibility of the three enzymes to dietary cholesterol  and cholate, and taurine induced CYP7A1 to produce its cholesterol-lowering  effect only in the presence of cholate in the cholesterol diet.	transcription
57678	2	335433	7	NULL	NULL	0	NULL	statement 1			produce					cholesterol-lowering effect					NULL		0	NULL	NULL	NULL	abs-batch0580-0599_life-sci_77_7_15936349_s_14	15936349	The overall results suggest that there are differences between  mice and rats in susceptibility of the three enzymes to dietary cholesterol  and cholate, and taurine induced CYP7A1 to produce its cholesterol-lowering  effect only in the presence of cholate in the cholesterol diet.	transcription
57679	3	335433	7	NULL	NULL	0	NULL	statement 2			in the presence of					cholate					NULL	cholesterol diet	0	NULL	NULL	NULL	abs-batch0580-0599_life-sci_77_7_15936349_s_14	15936349	The overall results suggest that there are differences between  mice and rats in susceptibility of the three enzymes to dietary cholesterol  and cholate, and taurine induced CYP7A1 to produce its cholesterol-lowering  effect only in the presence of cholate in the cholesterol diet.	transcription
78824	1	335434	6	NULL	NULL	NULL	NULL	chow	Chemical	feeding on	increases					HMG-CoA synthase mRNA	NucleicAcid	intestinal 			NULL	NPC1L1 null mice	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_32_33586_s_232	15173162	Intestinal HMG-CoA synthase mRNA was increased in both chow and cholesterol/cholate-fed NPC1L1 null mice, in contrast to NPC1L1 (+/-) and (+/+) mice, where HMG-CoA synthase was down-regulated with cholesterol/cholate feeding.	transcription
78825	2	335434	6	NULL	NULL	0	NULL	cholesterol/cholate	Chemical	feeding on	increases					HMG-CoA synthase mRNA	NucleicAcid				NULL	NPC1L1 null mice	0	NULL	NULL	NULL	gw70_jbiolchem_279_32_33586_s_232	15173162	Intestinal HMG-CoA synthase mRNA was increased in both chow and cholesterol/cholate-fed NPC1L1 null mice, in contrast to NPC1L1 (+/-) and (+/+) mice, where HMG-CoA synthase was down-regulated with cholesterol/cholate feeding.	transcription
57680	1	335434	7	NULL	NULL	0	NULL	HMG-CoA synthase mRNA		intestinal	is increased in					NPC1L1 null mice		chow-fed			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_32_33586_s_232	15173162	Intestinal HMG-CoA synthase mRNA was increased in both chow and cholesterol/cholate-fed NPC1L1 null mice, in contrast to NPC1L1 (+/-) and (+/+) mice, where HMG-CoA synthase was down-regulated with cholesterol/cholate feeding.	transcription
57681	2	335434	7	NULL	NULL	0	NULL	HMG-CoA synthase mRNA		intestinal	is increased in					NPC1L1 null mice		cholesterol/cholate-fed			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_32_33586_s_232	15173162	Intestinal HMG-CoA synthase mRNA was increased in both chow and cholesterol/cholate-fed NPC1L1 null mice, in contrast to NPC1L1 (+/-) and (+/+) mice, where HMG-CoA synthase was down-regulated with cholesterol/cholate feeding.	transcription
57682	3	335434	7	NULL	NULL	0	NULL	HMG-CoA synthase			is down-regulated in					NPC1L1 (+/-) mice		cholesterol/cholate-fed			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_32_33586_s_232	15173162	Intestinal HMG-CoA synthase mRNA was increased in both chow and cholesterol/cholate-fed NPC1L1 null mice, in contrast to NPC1L1 (+/-) and (+/+) mice, where HMG-CoA synthase was down-regulated with cholesterol/cholate feeding.	transcription
57683	4	335434	7	NULL	NULL	0	NULL	HMG-CoA synthase			is down-regulated in					NPC1L1 (+/+) mice		cholesterol/cholate-fed			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_32_33586_s_232	15173162	Intestinal HMG-CoA synthase mRNA was increased in both chow and cholesterol/cholate-fed NPC1L1 null mice, in contrast to NPC1L1 (+/-) and (+/+) mice, where HMG-CoA synthase was down-regulated with cholesterol/cholate feeding.	transcription
78826	1	335435	6	NULL	NULL	0	NULL	ABC	GP		is					ATP-binding cassette	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_3	15611112	Biliary cholesterol secretion is mediated by the ATP-binding cassette (ABC) transporters ABCG5 (G5) and ABCG8 (G8) and is stimulated by cholesterol and by the non-cholesterol steroids cholate and diosgenin.	transcription
78827	2	335435	6	NULL	NULL	0	NULL	ABCG5	GP		is a type of					ABC transporter	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_3	15611112	Biliary cholesterol secretion is mediated by the ATP-binding cassette (ABC) transporters ABCG5 (G5) and ABCG8 (G8) and is stimulated by cholesterol and by the non-cholesterol steroids cholate and diosgenin.	transcription
78828	3	335435	6	NULL	NULL	0	NULL	ABCG8	GP		is a type of					ABC transporter	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_3	15611112	Biliary cholesterol secretion is mediated by the ATP-binding cassette (ABC) transporters ABCG5 (G5) and ABCG8 (G8) and is stimulated by cholesterol and by the non-cholesterol steroids cholate and diosgenin.	transcription
78829	4	335435	6	NULL	NULL	0	NULL	ABCG5	GP		mediates					cholesterol	Chemical	secretion of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_3	15611112	Biliary cholesterol secretion is mediated by the ATP-binding cassette (ABC) transporters ABCG5 (G5) and ABCG8 (G8) and is stimulated by cholesterol and by the non-cholesterol steroids cholate and diosgenin.	transcription
78830	5	335435	6	NULL	NULL	0	NULL	ABCG8	GP		mediates					cholesterol	Chemical	secretion of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_3	15611112	Biliary cholesterol secretion is mediated by the ATP-binding cassette (ABC) transporters ABCG5 (G5) and ABCG8 (G8) and is stimulated by cholesterol and by the non-cholesterol steroids cholate and diosgenin.	transcription
78831	6	335435	6	NULL	NULL	0	NULL	diosgenin	Chemical		mediates					cholesterol	Chemical	secretion of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_3	15611112	Biliary cholesterol secretion is mediated by the ATP-binding cassette (ABC) transporters ABCG5 (G5) and ABCG8 (G8) and is stimulated by cholesterol and by the non-cholesterol steroids cholate and diosgenin.	transcription
57684	1	335435	7	NULL	NULL	0	NULL	ABCG5			mediates					Biliary cholesterol		secretion of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_3	15611112	Biliary cholesterol secretion is mediated by the ATP-binding cassette (ABC) transporters ABCG5 (G5) and ABCG8 (G8) and is stimulated by cholesterol and by the non-cholesterol steroids cholate and diosgenin.	transcription
57685	2	335435	7	NULL	NULL	0	NULL	ABCG8			mediates					Biliary cholesterol		secretion of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_3	15611112	Biliary cholesterol secretion is mediated by the ATP-binding cassette (ABC) transporters ABCG5 (G5) and ABCG8 (G8) and is stimulated by cholesterol and by the non-cholesterol steroids cholate and diosgenin.	transcription
57686	3	335435	7	NULL	NULL	0	NULL	ABC			is					ATP-binding cassette					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_3	15611112	Biliary cholesterol secretion is mediated by the ATP-binding cassette (ABC) transporters ABCG5 (G5) and ABCG8 (G8) and is stimulated by cholesterol and by the non-cholesterol steroids cholate and diosgenin.	transcription
57687	4	335435	7	NULL	NULL	0	NULL	ABCG5			is a type of					ABC transporter					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_3	15611112	Biliary cholesterol secretion is mediated by the ATP-binding cassette (ABC) transporters ABCG5 (G5) and ABCG8 (G8) and is stimulated by cholesterol and by the non-cholesterol steroids cholate and diosgenin.	transcription
57688	5	335435	7	NULL	NULL	0	NULL	ABCG8			is a type of					ABC transporter					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_3	15611112	Biliary cholesterol secretion is mediated by the ATP-binding cassette (ABC) transporters ABCG5 (G5) and ABCG8 (G8) and is stimulated by cholesterol and by the non-cholesterol steroids cholate and diosgenin.	transcription
57689	6	335435	7	NULL	NULL	0	NULL	cholate			stimulate					Biliary cholesterol		secretion of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_3	15611112	Biliary cholesterol secretion is mediated by the ATP-binding cassette (ABC) transporters ABCG5 (G5) and ABCG8 (G8) and is stimulated by cholesterol and by the non-cholesterol steroids cholate and diosgenin.	transcription
57690	7	335435	7	NULL	NULL	0	NULL	diosgenin			stimulate					Biliary cholesterol		secretion of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_3	15611112	Biliary cholesterol secretion is mediated by the ATP-binding cassette (ABC) transporters ABCG5 (G5) and ABCG8 (G8) and is stimulated by cholesterol and by the non-cholesterol steroids cholate and diosgenin.	transcription
57691	8	335435	7	NULL	NULL	0	NULL	cholate			is a type of					cholesterol steroid					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_3	15611112	Biliary cholesterol secretion is mediated by the ATP-binding cassette (ABC) transporters ABCG5 (G5) and ABCG8 (G8) and is stimulated by cholesterol and by the non-cholesterol steroids cholate and diosgenin.	transcription
57692	9	335435	7	NULL	NULL	0	NULL	 diosgenin			is a type of					non-cholesterol steroid					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_3	15611112	Biliary cholesterol secretion is mediated by the ATP-binding cassette (ABC) transporters ABCG5 (G5) and ABCG8 (G8) and is stimulated by cholesterol and by the non-cholesterol steroids cholate and diosgenin.	transcription
78974	1	335436	6	NULL	NULL	0	NULL	atherogenic diet			induces					hypercholesterolemia	MedicalFinding				NULL		0	NULL	NULL	NULL	gw70_amjpathol_163_6_2155_s_182	14633589	A cholate-containing high fat/high cholesterol atherogenic diet induces hypercholesterolemia and atherosclerosis in susceptible strains of mice including C57BL/6.	transcription
78975	2	335436	6	NULL	NULL	0	NULL	atherogenic diet			induces					atherosclerosis	MedicalFinding				NULL		0	NULL	NULL	NULL	gw70_amjpathol_163_6_2155_s_182	14633589	A cholate-containing high fat/high cholesterol atherogenic diet induces hypercholesterolemia and atherosclerosis in susceptible strains of mice including C57BL/6.	transcription
57693	1	335436	7	NULL	NULL	0	NULL	cholate-containing high fat/high cholesterol atherogenic diet			induce					hypercholesterolemia					NULL	C57BL/6 mice	0	NULL	NULL	NULL	gw70_amjpathol_163_6_2155_s_182	14633589	A cholate-containing high fat/high cholesterol atherogenic diet induces hypercholesterolemia and atherosclerosis in susceptible strains of mice including C57BL/6.	transcription
57694	2	335436	7	NULL	NULL	0	NULL	cholate-containing high fat/high cholesterol atherogenic diet			induce					atherosclerosis					NULL	C57BL/6 mice	0	NULL	NULL	NULL	gw70_amjpathol_163_6_2155_s_182	14633589	A cholate-containing high fat/high cholesterol atherogenic diet induces hypercholesterolemia and atherosclerosis in susceptible strains of mice including C57BL/6.	transcription
78976	1	335437	6	NULL	NULL	0	NULL	Inflammatory gene	GP	activation of	is dependent on					cholesterol	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_44_42774_s_218	12923166	Inflammatory gene activation was dependent on the presence of cholesterol in the diet, whereas the collagen gene family members were induced specifically by cholate.	transcription
78977	2	335437	6	NULL	NULL	0	NULL	cholate	Chemical		induces					collagen gene family members	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_44_42774_s_218	12923166	Inflammatory gene activation was dependent on the presence of cholesterol in the diet, whereas the collagen gene family members were induced specifically by cholate.	transcription
57696	1	335437	7	NULL	NULL	0	NULL	Inflammatory gene		activation of	depends on					cholesterol diet					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_44_42774_s_218	12923166	Inflammatory gene activation was dependent on the presence of cholesterol in the diet, whereas the collagen gene family members were induced specifically by cholate.	transcription
57697	2	335437	7	NULL	NULL	0	NULL	cholate			induce		specifically			collagen gene family					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_44_42774_s_218	12923166	Inflammatory gene activation was dependent on the presence of cholesterol in the diet, whereas the collagen gene family members were induced specifically by cholate.	transcription
57698	1	335438	7	NULL	NULL	0	NULL	cholate			stimulate					biliary cholesterol		secretion of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_202	15611112	Expression of G5 and G8 was required for the stimulation of biliary cholesterol secretion by either cholate or diosgenin, but the two choleretic agents activated G5G8-mediated cholesterol secretion by different mechanisms.	transcription
57699	2	335438	7	NULL	NULL	0	NULL	diosgenin			stimulate					biliary cholesterol		secretion of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_202	15611112	Expression of G5 and G8 was required for the stimulation of biliary cholesterol secretion by either cholate or diosgenin, but the two choleretic agents activated G5G8-mediated cholesterol secretion by different mechanisms.	transcription
57700	3	335438	7	NULL	NULL	0	NULL	G5		expression of	is required for					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_202	15611112	Expression of G5 and G8 was required for the stimulation of biliary cholesterol secretion by either cholate or diosgenin, but the two choleretic agents activated G5G8-mediated cholesterol secretion by different mechanisms.	transcription
57701	4	335438	7	NULL	NULL	0	NULL	G8		expression of	is required for					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_202	15611112	Expression of G5 and G8 was required for the stimulation of biliary cholesterol secretion by either cholate or diosgenin, but the two choleretic agents activated G5G8-mediated cholesterol secretion by different mechanisms.	transcription
57702	5	335438	7	NULL	NULL	0	NULL	G5		expression of	is required for					statement 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_202	15611112	Expression of G5 and G8 was required for the stimulation of biliary cholesterol secretion by either cholate or diosgenin, but the two choleretic agents activated G5G8-mediated cholesterol secretion by different mechanisms.	transcription
57703	6	335438	7	NULL	NULL	0	NULL	G8		expression of	is required for					statement 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_202	15611112	Expression of G5 and G8 was required for the stimulation of biliary cholesterol secretion by either cholate or diosgenin, but the two choleretic agents activated G5G8-mediated cholesterol secretion by different mechanisms.	transcription
57704	7	335438	7	NULL	NULL	0	NULL	G5G8			mediates					cholesterol		secretion of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_202	15611112	Expression of G5 and G8 was required for the stimulation of biliary cholesterol secretion by either cholate or diosgenin, but the two choleretic agents activated G5G8-mediated cholesterol secretion by different mechanisms.	transcription
57705	8	335438	7	NULL	NULL	0	NULL	cholate			activates					statement 7					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_202	15611112	Expression of G5 and G8 was required for the stimulation of biliary cholesterol secretion by either cholate or diosgenin, but the two choleretic agents activated G5G8-mediated cholesterol secretion by different mechanisms.	transcription
57706	9	335438	7	NULL	NULL	0	NULL	diosgenin			activates					statement 7					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_202	15611112	Expression of G5 and G8 was required for the stimulation of biliary cholesterol secretion by either cholate or diosgenin, but the two choleretic agents activated G5G8-mediated cholesterol secretion by different mechanisms.	transcription
57707	10	335438	7	NULL	NULL	0	NULL	cholate			is a type of					choleretic agents					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_202	15611112	Expression of G5 and G8 was required for the stimulation of biliary cholesterol secretion by either cholate or diosgenin, but the two choleretic agents activated G5G8-mediated cholesterol secretion by different mechanisms.	transcription
57708	11	335438	7	NULL	NULL	0	NULL	diosgenin			is a type of					choleretic agents					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_8742_s_202	15611112	Expression of G5 and G8 was required for the stimulation of biliary cholesterol secretion by either cholate or diosgenin, but the two choleretic agents activated G5G8-mediated cholesterol secretion by different mechanisms.	transcription
78978	1	335439	6	NULL	NULL	0	NULL	cholesterol	Chemical		induces					SAA gene	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_44_42774_s_159	12923166	The data above demonstrated that cholesterol was required for the large induction of SAA gene expression, whereas cholate was required for induction of collagen gene expression.	transcription
78979	2	335439	6	NULL	NULL	0	NULL	cholate	Chemical		induces					collagen gene	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_44_42774_s_159	12923166	The data above demonstrated that cholesterol was required for the large induction of SAA gene expression, whereas cholate was required for induction of collagen gene expression.	transcription
57709	1	335439	7	NULL	NULL	0	NULL	cholesterol			is required for					SAA gene		large induction of;;expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_44_42774_s_159	12923166	The data above demonstrated that cholesterol was required for the large induction of SAA gene expression, whereas cholate was required for induction of collagen gene expression.	transcription
57710	2	335439	7	NULL	NULL	0	NULL	cholate 			is required for					collagen gene		induction of;;expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_44_42774_s_159	12923166	The data above demonstrated that cholesterol was required for the large induction of SAA gene expression, whereas cholate was required for induction of collagen gene expression.	transcription
57711	1	335440	7	NULL	NULL	0	NULL	mice			express		constitutively			7alpha-hydroxylase gene		exogenous			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_1_126_s_180	9417056	Effect of cholate or cholestyramine on hepatic 7alpha-hydroxylase activity and plasma LDL cholesterol concentrations in LDL receptor /  mice constitutively expressing an exogenous 7alpha-hydroxylase gene.	transcription
57712	1	335441	7	NULL	NULL	0	NULL	cholate			does not induce					collagen family member					NULL	C57BL/6ByJ mice	0	NULL	NULL	NULL	gw70_jbiolchem_278_44_42774_s_197	12923166	Thus, the two C57BL/6 substrains differ substantially in their gene expression response to dietary cholesterol, and C57BL/6ByJ mice also fail to induce collagen family members to the levels seen in C57BL/6J mice in response to cholate.	transcription
57713	2	335441	7	NULL	NULL	0	NULL	cholate			 induce					collagen family member					NULL	C57BL/6J mice	0	NULL	NULL	NULL	gw70_jbiolchem_278_44_42774_s_197	12923166	Thus, the two C57BL/6 substrains differ substantially in their gene expression response to dietary cholesterol, and C57BL/6ByJ mice also fail to induce collagen family members to the levels seen in C57BL/6J mice in response to cholate.	transcription
57714	1	335442	7	NULL	NULL	0	NULL	 SR-BI			facilitate					atherosclerosis					NULL	LDLr - / - mice	0	NULL	NULL	NULL	gw70_amjpathol_165_3_785_s_129	15331403	Because SR-BI facilitated atherosclerosis in LDLr - / -  mice after only 4 weeks of Western-type diet feeding, in contrast to the protective role at 9 and 12 weeks, this prompted us to study the effect in a second model of atherosclerosis with small fatty streak lesions: WT mice on a high-cholesterol/cholate diet.	transcription
78980	1	335446	6	NULL	NULL	0	NULL	LDLr	GP		facilitates					foam cell	cell	formation of 			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_8_1961_s_180	10938018	13  Although different animal models were used to analyze diet-induced (with and without the addition of cholate) atherosclerosis in these studies, which could make direct comparisons difficult, the present data strongly suggest that the LDLr can facilitate foam cell formation only under conditions of moderate cholesterol levels.	transcription
78981	2	335446	6	NULL	NULL	0	NULL	statement 1	Process		occurs under					cholesterol levels	Chemical	moderate			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_8_1961_s_180	10938018	13  Although different animal models were used to analyze diet-induced (with and without the addition of cholate) atherosclerosis in these studies, which could make direct comparisons difficult, the present data strongly suggest that the LDLr can facilitate foam cell formation only under conditions of moderate cholesterol levels.	transcription
57715	1	335446	7	NULL	NULL	0	NULL	LDLr			facilitate		could			foam cell		formation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_8_1961_s_180	10938018	13  Although different animal models were used to analyze diet-induced (with and without the addition of cholate) atherosclerosis in these studies, which could make direct comparisons difficult, the present data strongly suggest that the LDLr can facilitate foam cell formation only under conditions of moderate cholesterol levels.	transcription
57716	2	335446	7	NULL	NULL	0	NULL	statement 1			under conditions of					cholesterol		moderate			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_20_8_1961_s_180	10938018	13  Although different animal models were used to analyze diet-induced (with and without the addition of cholate) atherosclerosis in these studies, which could make direct comparisons difficult, the present data strongly suggest that the LDLr can facilitate foam cell formation only under conditions of moderate cholesterol levels.	transcription
57717	1	335447	7	NULL	NULL	0	NULL	 dietary cholate			elevates					RIP140		expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_20_15482_s_260	10809780	The marked elevation of RIP140 expression induced by dietary cholate also suggested a bile acid/FXR-mediated feedback regulation at the feed-forward stage of cholesterol disposal, in addition to direct repression of Cyp7a through  cis-acting elements in the  cyp7a gene ( 37).	transcription
57718	2	335447	7	NULL	NULL	0	NULL	bile acid			mediates					feedback regulation					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_20_15482_s_260	10809780	The marked elevation of RIP140 expression induced by dietary cholate also suggested a bile acid/FXR-mediated feedback regulation at the feed-forward stage of cholesterol disposal, in addition to direct repression of Cyp7a through  cis-acting elements in the  cyp7a gene ( 37).	transcription
57719	3	335447	7	NULL	NULL	0	NULL	FXR			mediates					feedback regulation					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_20_15482_s_260	10809780	The marked elevation of RIP140 expression induced by dietary cholate also suggested a bile acid/FXR-mediated feedback regulation at the feed-forward stage of cholesterol disposal, in addition to direct repression of Cyp7a through  cis-acting elements in the  cyp7a gene ( 37).	transcription
57720	4	335447	7	NULL	NULL	0	NULL	statement 2			occur during					cholesterol		feed-forward stage of;;disposal of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_20_15482_s_260	10809780	The marked elevation of RIP140 expression induced by dietary cholate also suggested a bile acid/FXR-mediated feedback regulation at the feed-forward stage of cholesterol disposal, in addition to direct repression of Cyp7a through  cis-acting elements in the  cyp7a gene ( 37).	transcription
57721	5	335447	7	NULL	NULL	0	NULL	statement 3			occur during					cholesterol		feed-forward stage of;;disposal of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_20_15482_s_260	10809780	The marked elevation of RIP140 expression induced by dietary cholate also suggested a bile acid/FXR-mediated feedback regulation at the feed-forward stage of cholesterol disposal, in addition to direct repression of Cyp7a through  cis-acting elements in the  cyp7a gene ( 37).	transcription
57722	6	335447	7	NULL	NULL	0	NULL	 cyp7a gene			repress		directly	cis-acting elements		Cyp7a					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_20_15482_s_260	10809780	The marked elevation of RIP140 expression induced by dietary cholate also suggested a bile acid/FXR-mediated feedback regulation at the feed-forward stage of cholesterol disposal, in addition to direct repression of Cyp7a through  cis-acting elements in the  cyp7a gene ( 37).	transcription
57723	7	335447	7	NULL	NULL	0	NULL	statement 1			suggest					statement 4					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_20_15482_s_260	10809780	The marked elevation of RIP140 expression induced by dietary cholate also suggested a bile acid/FXR-mediated feedback regulation at the feed-forward stage of cholesterol disposal, in addition to direct repression of Cyp7a through  cis-acting elements in the  cyp7a gene ( 37).	transcription
57724	8	335447	7	NULL	NULL	0	NULL	statement 1			suggest					statement 5					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_20_15482_s_260	10809780	The marked elevation of RIP140 expression induced by dietary cholate also suggested a bile acid/FXR-mediated feedback regulation at the feed-forward stage of cholesterol disposal, in addition to direct repression of Cyp7a through  cis-acting elements in the  cyp7a gene ( 37).	transcription
57725	9	335447	7	NULL	NULL	0	NULL	statement 1			suggest					statement 6					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_20_15482_s_260	10809780	The marked elevation of RIP140 expression induced by dietary cholate also suggested a bile acid/FXR-mediated feedback regulation at the feed-forward stage of cholesterol disposal, in addition to direct repression of Cyp7a through  cis-acting elements in the  cyp7a gene ( 37).	transcription
57726	1	335448	7	NULL	NULL	0	NULL	high-cholesterol diet			elevates					transaminase		liver			NULL	mice	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_8_1960_s_24	10446078	10  Although no murine model fully recapitulates all of the features of human atherosclerosis, a potential drawback to using mice fed a high-fat, high-cholesterol, cholate-containing diet is that the diet itself is inflammatory when fed to certain strains of mice, and results in liver transaminase elevations, activation of hepatic NFkappaB, increases in acute-phase reactants such as serum amyloid A, and liberation of inflammatory cytokines.	transcription
57727	2	335448	7	NULL	NULL	0	NULL	high-cholesterol diet			activates					NFkappaB		hepatic			NULL	mice	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_8_1960_s_24	10446078	10  Although no murine model fully recapitulates all of the features of human atherosclerosis, a potential drawback to using mice fed a high-fat, high-cholesterol, cholate-containing diet is that the diet itself is inflammatory when fed to certain strains of mice, and results in liver transaminase elevations, activation of hepatic NFkappaB, increases in acute-phase reactants such as serum amyloid A, and liberation of inflammatory cytokines.	transcription
57728	3	335448	7	NULL	NULL	0	NULL	high-cholesterol diet			increase					serum amyloid A					NULL	mice	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_8_1960_s_24	10446078	10  Although no murine model fully recapitulates all of the features of human atherosclerosis, a potential drawback to using mice fed a high-fat, high-cholesterol, cholate-containing diet is that the diet itself is inflammatory when fed to certain strains of mice, and results in liver transaminase elevations, activation of hepatic NFkappaB, increases in acute-phase reactants such as serum amyloid A, and liberation of inflammatory cytokines.	transcription
57729	4	335448	7	NULL	NULL	0	NULL	high-cholesterol diet			increase					inflammatory cytokines		liberation of			NULL	mice	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_8_1960_s_24	10446078	10  Although no murine model fully recapitulates all of the features of human atherosclerosis, a potential drawback to using mice fed a high-fat, high-cholesterol, cholate-containing diet is that the diet itself is inflammatory when fed to certain strains of mice, and results in liver transaminase elevations, activation of hepatic NFkappaB, increases in acute-phase reactants such as serum amyloid A, and liberation of inflammatory cytokines.	transcription
57730	5	335448	7	NULL	NULL	0	NULL	cholate-containing diet			elevates					transaminase		liver			NULL	mice	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_8_1960_s_24	10446078	10  Although no murine model fully recapitulates all of the features of human atherosclerosis, a potential drawback to using mice fed a high-fat, high-cholesterol, cholate-containing diet is that the diet itself is inflammatory when fed to certain strains of mice, and results in liver transaminase elevations, activation of hepatic NFkappaB, increases in acute-phase reactants such as serum amyloid A, and liberation of inflammatory cytokines.	transcription
57731	6	335448	7	NULL	NULL	0	NULL	cholate-containing diet			activates					NFkappaB		hepatic			NULL	mice	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_8_1960_s_24	10446078	10  Although no murine model fully recapitulates all of the features of human atherosclerosis, a potential drawback to using mice fed a high-fat, high-cholesterol, cholate-containing diet is that the diet itself is inflammatory when fed to certain strains of mice, and results in liver transaminase elevations, activation of hepatic NFkappaB, increases in acute-phase reactants such as serum amyloid A, and liberation of inflammatory cytokines.	transcription
57732	7	335448	7	NULL	NULL	0	NULL	cholate-containing diet			increase					serum amyloid A					NULL	mice	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_8_1960_s_24	10446078	10  Although no murine model fully recapitulates all of the features of human atherosclerosis, a potential drawback to using mice fed a high-fat, high-cholesterol, cholate-containing diet is that the diet itself is inflammatory when fed to certain strains of mice, and results in liver transaminase elevations, activation of hepatic NFkappaB, increases in acute-phase reactants such as serum amyloid A, and liberation of inflammatory cytokines.	transcription
57733	8	335448	7	NULL	NULL	0	NULL	cholate-containing diet			increase					inflammatory cytokines		liberation of			NULL	mice	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_8_1960_s_24	10446078	10  Although no murine model fully recapitulates all of the features of human atherosclerosis, a potential drawback to using mice fed a high-fat, high-cholesterol, cholate-containing diet is that the diet itself is inflammatory when fed to certain strains of mice, and results in liver transaminase elevations, activation of hepatic NFkappaB, increases in acute-phase reactants such as serum amyloid A, and liberation of inflammatory cytokines.	transcription
78982	1	335452	6	NULL	NULL	0	NULL	Cbp1	GP		bind					COB	GP			CCG region of UTR	NULL		0	NULL	NULL	NULL	gw70_genetics_171_3_949_s_26	16118200	Recovery of a dominant suppressor in  CBP1 that suppresses the  ACG mutation supports the hypothesis that Cbp1 interacts with the CCG region of the  COB 5''-UTR.	transcription
57734	1	335452	7	NULL	NULL	0	NULL	Cbp1			interacts with					COB				CCG region of the 5''-UTR	NULL		0	NULL	NULL	NULL	gw70_genetics_171_3_949_s_26	16118200	Recovery of a dominant suppressor in  CBP1 that suppresses the  ACG mutation supports the hypothesis that Cbp1 interacts with the CCG region of the  COB 5''-UTR.	transcription
57735	2	335452	7	NULL	NULL	0	NULL	CBP1 		dominant suppressor in	suppress							mutation		 ACG 	NULL		0	NULL	NULL	NULL	gw70_genetics_171_3_949_s_26	16118200	Recovery of a dominant suppressor in  CBP1 that suppresses the  ACG mutation supports the hypothesis that Cbp1 interacts with the CCG region of the  COB 5''-UTR.	transcription
57736	3	335452	7	NULL	NULL	0	NULL	statement 2			support					statement 1					NULL		0	NULL	NULL	NULL	gw70_genetics_171_3_949_s_26	16118200	Recovery of a dominant suppressor in  CBP1 that suppresses the  ACG mutation supports the hypothesis that Cbp1 interacts with the CCG region of the  COB 5''-UTR.	transcription
57737	1	335453	7	NULL	NULL	0	NULL	adenosylcobalamin			reacts with			Cys 408		coenzyme B12					NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_70_0_121_s_362	11395404	Radical chemistry is projected into the substrate binding site from adenosylcobalamin  through Cys 408, which reacts with coenzyme B12 to produce cob(II)alamin, 5''-deoxyadenosine, and the Cys 408-thiyl radical.	transcription
57738	2	335453	7	NULL	NULL	0	NULL	statement 1			produce					cob(II)alamin, 5''-deoxyadenosine					NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_70_0_121_s_362	11395404	Radical chemistry is projected into the substrate binding site from adenosylcobalamin  through Cys 408, which reacts with coenzyme B12 to produce cob(II)alamin, 5''-deoxyadenosine, and the Cys 408-thiyl radical.	transcription
57739	3	335453	7	NULL	NULL	0	NULL	statement 1			produce								Cys 408-thiyl radical		NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_70_0_121_s_362	11395404	Radical chemistry is projected into the substrate binding site from adenosylcobalamin  through Cys 408, which reacts with coenzyme B12 to produce cob(II)alamin, 5''-deoxyadenosine, and the Cys 408-thiyl radical.	transcription
57740	1	335454	7	NULL	NULL	0	NULL				is present at				CCG trinucleotide	COB mRNA		mature		11 nucleotides downstream of the 5' end 	NULL	yeast strains with mutations in the AU-rich COB 5'' UTR	NULL	NULL	NULL	NULL	gw70_molbiolcell_15_6_2674_s_21	15047869	Analyses of yeast strains with mutations in the AU-rich  COB 5'' UTR have shown that a CCG trinucleotide 11 nucleotides downstream of the 5' end of the mature mRNA plays a key role in the interaction with Cbp1; mutations that change this sequence to  ACG, CC U, or C AG result in decreased stability of the  COB mRNA (Chen and Dieckmann, 1997 ).	transcription
57741	2	335454	7	NULL	NULL	0	NULL				plays a key role in				CCG trinucleotide	Cbp1		interaction with			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_6_2674_s_21	15047869	Analyses of yeast strains with mutations in the AU-rich  COB 5'' UTR have shown that a CCG trinucleotide 11 nucleotides downstream of the 5' end of the mature mRNA plays a key role in the interaction with Cbp1; mutations that change this sequence to  ACG, CC U, or C AG result in decreased stability of the  COB mRNA (Chen and Dieckmann, 1997 ).	transcription
57742	3	335454	7	NULL	NULL	0	NULL				mutated to				CCG trinucleotide					 ACG	NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_6_2674_s_21	15047869	Analyses of yeast strains with mutations in the AU-rich  COB 5'' UTR have shown that a CCG trinucleotide 11 nucleotides downstream of the 5' end of the mature mRNA plays a key role in the interaction with Cbp1; mutations that change this sequence to  ACG, CC U, or C AG result in decreased stability of the  COB mRNA (Chen and Dieckmann, 1997 ).	transcription
57743	4	335454	7	NULL	NULL	0	NULL				mutated to				CCG trinucleotide					CC U	NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_6_2674_s_21	15047869	Analyses of yeast strains with mutations in the AU-rich  COB 5'' UTR have shown that a CCG trinucleotide 11 nucleotides downstream of the 5' end of the mature mRNA plays a key role in the interaction with Cbp1; mutations that change this sequence to  ACG, CC U, or C AG result in decreased stability of the  COB mRNA (Chen and Dieckmann, 1997 ).	transcription
57744	5	335454	7	NULL	NULL	0	NULL				mutated to				CCG trinucleotide					C AG	NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_6_2674_s_21	15047869	Analyses of yeast strains with mutations in the AU-rich  COB 5'' UTR have shown that a CCG trinucleotide 11 nucleotides downstream of the 5' end of the mature mRNA plays a key role in the interaction with Cbp1; mutations that change this sequence to  ACG, CC U, or C AG result in decreased stability of the  COB mRNA (Chen and Dieckmann, 1997 ).	transcription
57745	6	335454	7	NULL	NULL	0	NULL	statement 3			result in					COB mRNA		decreased stability of			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_6_2674_s_21	15047869	Analyses of yeast strains with mutations in the AU-rich  COB 5'' UTR have shown that a CCG trinucleotide 11 nucleotides downstream of the 5' end of the mature mRNA plays a key role in the interaction with Cbp1; mutations that change this sequence to  ACG, CC U, or C AG result in decreased stability of the  COB mRNA (Chen and Dieckmann, 1997 ).	transcription
57746	7	335454	7	NULL	NULL	0	NULL	statement 4			result in					COB mRNA		decreased stability of			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_6_2674_s_21	15047869	Analyses of yeast strains with mutations in the AU-rich  COB 5'' UTR have shown that a CCG trinucleotide 11 nucleotides downstream of the 5' end of the mature mRNA plays a key role in the interaction with Cbp1; mutations that change this sequence to  ACG, CC U, or C AG result in decreased stability of the  COB mRNA (Chen and Dieckmann, 1997 ).	transcription
57747	8	335454	7	NULL	NULL	0	NULL	statement 5			result in					COB mRNA		decreased stability of			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_15_6_2674_s_21	15047869	Analyses of yeast strains with mutations in the AU-rich  COB 5'' UTR have shown that a CCG trinucleotide 11 nucleotides downstream of the 5' end of the mature mRNA plays a key role in the interaction with Cbp1; mutations that change this sequence to  ACG, CC U, or C AG result in decreased stability of the  COB mRNA (Chen and Dieckmann, 1997 ).	transcription
78983	1	335455	6	NULL	NULL	0	NULL	Co(II)	Chemical		is reduced to					Co(I)	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_49_40948_s_32	16207720	As mentioned above, we previously hypothesized that FldA reduces Co(II) to Co(I) in the CobA active site, triggering the attack of the Co(I) nucleophile on the 5' carbon of the ribosyl moiety of ATP ( ).	transcription
78984	2	335455	6	NULL	NULL	0	NULL	FldA	GP		play a role in					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_49_40948_s_32	16207720	As mentioned above, we previously hypothesized that FldA reduces Co(II) to Co(I) in the CobA active site, triggering the attack of the Co(I) nucleophile on the 5' carbon of the ribosyl moiety of ATP ( ).	transcription
57748	1	335455	7	NULL	NULL	0	NULL	Co(II)			converted to					Co(I)			CobA active site		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_49_40948_s_32	16207720	As mentioned above, we previously hypothesized that FldA reduces Co(II) to Co(I) in the CobA active site, triggering the attack of the Co(I) nucleophile on the 5' carbon of the ribosyl moiety of ATP ( ).	transcription
57749	2	335455	7	NULL	NULL	0	NULL	FldA			reduces					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_49_40948_s_32	16207720	As mentioned above, we previously hypothesized that FldA reduces Co(II) to Co(I) in the CobA active site, triggering the attack of the Co(I) nucleophile on the 5' carbon of the ribosyl moiety of ATP ( ).	transcription
57750	3	335455	7	NULL	NULL	0	NULL	Co(I) nucleophile			attack					ATP			5' carbon of the ribosyl moiety 		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_49_40948_s_32	16207720	As mentioned above, we previously hypothesized that FldA reduces Co(II) to Co(I) in the CobA active site, triggering the attack of the Co(I) nucleophile on the 5' carbon of the ribosyl moiety of ATP ( ).	transcription
57751	4	335455	7	NULL	NULL	0	NULL	statement 2			triggers					statement 3					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_49_40948_s_32	16207720	As mentioned above, we previously hypothesized that FldA reduces Co(II) to Co(I) in the CobA active site, triggering the attack of the Co(I) nucleophile on the 5' carbon of the ribosyl moiety of ATP ( ).	transcription
78985	1	335457	6	NULL	NULL	0	NULL	GTP	Chemical		does not increase					CobU	GP	activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_36_27576_s_265	10869342	The addition of GTP to the ATP:AdoCbi kinase reaction after 30 min did not restore the reaction rate to the level seen when GTP was added at the start of the reaction (Fig.  5), suggesting that GTP could no longer increase the activity of CobU.	transcription
59041	1	335457	7	NULL	NULL	0	NULL	GTP			does not increase					CobU		activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_36_27576_s_265	10869342	The addition of GTP to the ATP:AdoCbi kinase reaction after 30 min did not restore the reaction rate to the level seen when GTP was added at the start of the reaction (Fig.  5), suggesting that GTP could no longer increase the activity of CobU.	transcription
78986	1	335458	6	NULL	NULL	NULL	NULL	PD98059	Chemical		is a type of					MEK inhibitor	GP				NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_139_3_475_s_162	12788807	We used PD98059 (IC50=5 - 10  muM), a highly selective MEK inhibitor that binds to the inactive forms of MEK and prevents its activation by upstream activators (English & Cobb, 2002  ).	transcription
59042	1	335458	7	NULL	NULL	0	NULL	MEK inhibitor		highly selective	bind					MEK		inactive			NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_139_3_475_s_162	12788807	We used PD98059 (IC50=5 - 10  muM), a highly selective MEK inhibitor that binds to the inactive forms of MEK and prevents its activation by upstream activators (English & Cobb, 2002  ).	transcription
59043	2	335458	7	NULL	NULL	0	NULL	statement 1			prevent					upstream activators		activation by			NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_139_3_475_s_162	12788807	We used PD98059 (IC50=5 - 10  muM), a highly selective MEK inhibitor that binds to the inactive forms of MEK and prevents its activation by upstream activators (English & Cobb, 2002  ).	transcription
78987	1	335463	6	NULL	NULL	0	NULL	guanosine phosphorylase	GP		catalyzes					purine bases	Chemical	recycling of 			NULL		0	NULL	NULL	NULL	gw70_annurevplantbiol_57_0_805_s_421	16669783	Another route to recycle purine bases is catalyzed by adenine  or inosine/guanosine phosphorylases.	transcription
78988	2	335463	6	NULL	NULL	0	NULL	inosine phosphorylase	GP		catalyzes					purine bases	Chemical	recycling of 			NULL		0	NULL	NULL	NULL	gw70_annurevplantbiol_57_0_805_s_421	16669783	Another route to recycle purine bases is catalyzed by adenine  or inosine/guanosine phosphorylases.	transcription
59044	1	335463	7	NULL	NULL	0	NULL	adenine phosphorylase			catalyze					purine bases		recycling of			NULL		NULL	NULL	NULL	NULL	gw70_annurevplantbiol_57_0_805_s_421	16669783	Another route to recycle purine bases is catalyzed by adenine  or inosine/guanosine phosphorylases.	transcription
59045	2	335463	7	NULL	NULL	0	NULL	 inosine phosphorylase			catalyze					purine bases		recycling of			NULL		NULL	NULL	NULL	NULL	gw70_annurevplantbiol_57_0_805_s_421	16669783	Another route to recycle purine bases is catalyzed by adenine  or inosine/guanosine phosphorylases.	transcription
59046	3	335463	7	NULL	NULL	0	NULL	guanosine phosphorylase			catalyze					purine bases		recycling of			NULL		0	NULL	NULL	NULL	gw70_annurevplantbiol_57_0_805_s_421	16669783	Another route to recycle purine bases is catalyzed by adenine  or inosine/guanosine phosphorylases.	transcription
59047	4	335463	7	NULL	NULL	0	NULL	statement 1			is an alternative to					statement 2					NULL		0	NULL	NULL	NULL	gw70_annurevplantbiol_57_0_805_s_421	16669783	Another route to recycle purine bases is catalyzed by adenine  or inosine/guanosine phosphorylases.	transcription
59048	5	335463	7	NULL	NULL	0	NULL	statement 1			is an alternative to					statement 3					NULL		0	NULL	NULL	NULL	gw70_annurevplantbiol_57_0_805_s_421	16669783	Another route to recycle purine bases is catalyzed by adenine  or inosine/guanosine phosphorylases.	transcription
59049	1	335464	7	NULL	NULL	0	NULL	 inosine			inhibit		specifically			P1					NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_29_5_987_s_18	16040150	They identified two high-affinity adenosine  transporters, designated P1 and P2, which could be specifically inhibited by inosine  and adenine, respectively   .	transcription
59050	2	335464	7	NULL	NULL	0	NULL	adenine 			inhibit		specifically			P2					NULL		NULL	NULL	NULL	NULL	gw70_femsmicrobiolrev_29_5_987_s_18	16040150	They identified two high-affinity adenosine  transporters, designated P1 and P2, which could be specifically inhibited by inosine  and adenine, respectively   .	transcription
59051	3	335464	7	NULL	NULL	0	NULL	P1			is a type of					adenosine transporter		high-affinity			NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_29_5_987_s_18	16040150	They identified two high-affinity adenosine  transporters, designated P1 and P2, which could be specifically inhibited by inosine  and adenine, respectively   .	transcription
59052	4	335464	7	NULL	NULL	0	NULL	P2			is a type of					adenosine transporter		high-affinity			NULL		0	NULL	NULL	NULL	gw70_femsmicrobiolrev_29_5_987_s_18	16040150	They identified two high-affinity adenosine  transporters, designated P1 and P2, which could be specifically inhibited by inosine  and adenine, respectively   .	transcription
78989	1	335465	6	NULL	NULL	0	NULL	inosine	Chemical		inhibits					adenosine	Chemical	uptake of 			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_56_6_1162_s_76	10570043	Conversely, inosine completely inhibited [3]adenosine uptake in the presence of 100 muM adenine (not shown).	transcription
59053	1	335465	7	NULL	NULL	0	NULL	inosine			inhibit		completely			adenosine		uptake of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_56_6_1162_s_76	10570043	Conversely, inosine completely inhibited [3]adenosine uptake in the presence of 100 muM adenine (not shown).	transcription
59054	2	335465	7	NULL	NULL	0	NULL	statement 1			in the presence of					adenine					NULL		0	NULL	NULL	NULL	gw60_molpharmacol_56_6_1162_s_76	10570043	Conversely, inosine completely inhibited [3]adenosine uptake in the presence of 100 muM adenine (not shown).	transcription
78990	1	335466	6	NULL	NULL	0	NULL	P1 system	GP		is inhibited by					inosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_16_9486_s_21	9545276	The P1 system was selectively inhibited by inosine, whereas the P2 transporter was specifically blocked by adenine.	transcription
78991	2	335466	6	NULL	NULL	0	NULL	P2 transporter	GP		is blocked by					adenine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_16_9486_s_21	9545276	The P1 system was selectively inhibited by inosine, whereas the P2 transporter was specifically blocked by adenine.	transcription
59055	1	335466	7	NULL	NULL	0	NULL	inosine			inhibit		selectively			P1 system					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_16_9486_s_21	9545276	The P1 system was selectively inhibited by inosine, whereas the P2 transporter was specifically blocked by adenine.	transcription
59056	2	335466	7	NULL	NULL	0	NULL	adenine			blocks		specifically			P2 transporter					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_16_9486_s_21	9545276	The P1 system was selectively inhibited by inosine, whereas the P2 transporter was specifically blocked by adenine.	transcription
59057	1	335467	7	NULL	NULL	0	NULL	fructose			induce					adenine nucleotides		degradation of			NULL	humans	0	NULL	NULL	NULL	abs-batch0720-0739_clin-chem_32_5_3698269_s_1	3698269	Liquid-chromatographic measurements of inosine, hypoxanthine, and xanthine in studies of fructose-induced degradation of adenine nucleotides in humans and rats..	transcription
59058	2	335467	7	NULL	NULL	0	NULL	fructose			induce					adenine nucleotides		degradation of			NULL	rats	0	NULL	NULL	NULL	abs-batch0720-0739_clin-chem_32_5_3698269_s_1	3698269	Liquid-chromatographic measurements of inosine, hypoxanthine, and xanthine in studies of fructose-induced degradation of adenine nucleotides in humans and rats..	transcription
78992	1	335468	6	NULL	NULL	0	NULL	dCTP	Chemical		is formed from					dUTP	Chemical				NULL		0	NULL	NULL	NULL	gw60_chembiol_9_2_245_s_64	11880039	URA7 is a CTP synthase that catalyzes the formation of dCTP from dUTP, the final step in pyrimidine biosynthesis, whereas AAH1 is an adenine deaminase (adenine aminohydrolase), an enzyme of the purine salvage pathway, and converts adenosine to inosine     [33-36]  .	transcription
78993	2	335468	6	NULL	NULL	0	NULL	URA7	GP		catalyzes					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_chembiol_9_2_245_s_64	11880039	URA7 is a CTP synthase that catalyzes the formation of dCTP from dUTP, the final step in pyrimidine biosynthesis, whereas AAH1 is an adenine deaminase (adenine aminohydrolase), an enzyme of the purine salvage pathway, and converts adenosine to inosine     [33-36]  .	transcription
78994	3	335468	6	NULL	NULL	0	NULL	URA7	GP		is a type of					CTP synthase	GP				NULL		0	NULL	NULL	NULL	gw60_chembiol_9_2_245_s_64	11880039	URA7 is a CTP synthase that catalyzes the formation of dCTP from dUTP, the final step in pyrimidine biosynthesis, whereas AAH1 is an adenine deaminase (adenine aminohydrolase), an enzyme of the purine salvage pathway, and converts adenosine to inosine     [33-36]  .	transcription
78995	4	335468	6	NULL	NULL	0	NULL	AAH1	GP		is					adenine deaminase	GP				NULL		0	NULL	NULL	NULL	gw60_chembiol_9_2_245_s_64	11880039	URA7 is a CTP synthase that catalyzes the formation of dCTP from dUTP, the final step in pyrimidine biosynthesis, whereas AAH1 is an adenine deaminase (adenine aminohydrolase), an enzyme of the purine salvage pathway, and converts adenosine to inosine     [33-36]  .	transcription
78996	5	335468	6	NULL	NULL	0	NULL	adenosine	Chemical		is converted to					inosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_chembiol_9_2_245_s_64	11880039	URA7 is a CTP synthase that catalyzes the formation of dCTP from dUTP, the final step in pyrimidine biosynthesis, whereas AAH1 is an adenine deaminase (adenine aminohydrolase), an enzyme of the purine salvage pathway, and converts adenosine to inosine     [33-36]  .	transcription
78997	6	335468	6	NULL	NULL	0	NULL	AAH1	GP		catalyzes					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_chembiol_9_2_245_s_64	11880039	URA7 is a CTP synthase that catalyzes the formation of dCTP from dUTP, the final step in pyrimidine biosynthesis, whereas AAH1 is an adenine deaminase (adenine aminohydrolase), an enzyme of the purine salvage pathway, and converts adenosine to inosine     [33-36]  .	transcription
59059	1	335468	7	NULL	NULL	0	NULL	dUTP			converted to					dCTP					NULL		0	NULL	NULL	NULL	gw60_chembiol_9_2_245_s_64	11880039	URA7 is a CTP synthase that catalyzes the formation of dCTP from dUTP, the final step in pyrimidine biosynthesis, whereas AAH1 is an adenine deaminase (adenine aminohydrolase), an enzyme of the purine salvage pathway, and converts adenosine to inosine     [33-36]  .	transcription
59060	2	335468	7	NULL	NULL	0	NULL	URA7			catalyze					statement 1					NULL		0	NULL	NULL	NULL	gw60_chembiol_9_2_245_s_64	11880039	URA7 is a CTP synthase that catalyzes the formation of dCTP from dUTP, the final step in pyrimidine biosynthesis, whereas AAH1 is an adenine deaminase (adenine aminohydrolase), an enzyme of the purine salvage pathway, and converts adenosine to inosine     [33-36]  .	transcription
59061	3	335468	7	NULL	NULL	0	NULL	URA7			is a type of					CTP synthase					NULL		0	NULL	NULL	NULL	gw60_chembiol_9_2_245_s_64	11880039	URA7 is a CTP synthase that catalyzes the formation of dCTP from dUTP, the final step in pyrimidine biosynthesis, whereas AAH1 is an adenine deaminase (adenine aminohydrolase), an enzyme of the purine salvage pathway, and converts adenosine to inosine     [33-36]  .	transcription
59062	4	335468	7	NULL	NULL	0	NULL	statement 1			final step in					pyrimidine		biosynthesis of			NULL		0	NULL	NULL	NULL	gw60_chembiol_9_2_245_s_64	11880039	URA7 is a CTP synthase that catalyzes the formation of dCTP from dUTP, the final step in pyrimidine biosynthesis, whereas AAH1 is an adenine deaminase (adenine aminohydrolase), an enzyme of the purine salvage pathway, and converts adenosine to inosine     [33-36]  .	transcription
59063	5	335468	7	NULL	NULL	0	NULL	AAH1			is a type of					adenine deaminase					NULL		NULL	NULL	NULL	NULL	gw60_chembiol_9_2_245_s_64	11880039	URA7 is a CTP synthase that catalyzes the formation of dCTP from dUTP, the final step in pyrimidine biosynthesis, whereas AAH1 is an adenine deaminase (adenine aminohydrolase), an enzyme of the purine salvage pathway, and converts adenosine to inosine     [33-36]  .	transcription
59064	6	335468	7	NULL	NULL	0	NULL	AAH1			is 					adenine aminohydrolase					NULL		NULL	NULL	NULL	NULL	gw60_chembiol_9_2_245_s_64	11880039	URA7 is a CTP synthase that catalyzes the formation of dCTP from dUTP, the final step in pyrimidine biosynthesis, whereas AAH1 is an adenine deaminase (adenine aminohydrolase), an enzyme of the purine salvage pathway, and converts adenosine to inosine     [33-36]  .	transcription
59065	7	335468	7	NULL	NULL	0	NULL	adenosine			converted to					inosine					NULL		0	NULL	NULL	NULL	gw60_chembiol_9_2_245_s_64	11880039	URA7 is a CTP synthase that catalyzes the formation of dCTP from dUTP, the final step in pyrimidine biosynthesis, whereas AAH1 is an adenine deaminase (adenine aminohydrolase), an enzyme of the purine salvage pathway, and converts adenosine to inosine     [33-36]  .	transcription
59066	8	335468	7	NULL	NULL	0	NULL	AAH1			converts					statement 7					NULL		0	NULL	NULL	NULL	gw60_chembiol_9_2_245_s_64	11880039	URA7 is a CTP synthase that catalyzes the formation of dCTP from dUTP, the final step in pyrimidine biosynthesis, whereas AAH1 is an adenine deaminase (adenine aminohydrolase), an enzyme of the purine salvage pathway, and converts adenosine to inosine     [33-36]  .	transcription
59067	9	335468	7	NULL	NULL	0	NULL	AAH1			is an enzyme of					 purine salvage pathway					NULL		0	NULL	NULL	NULL	gw60_chembiol_9_2_245_s_64	11880039	URA7 is a CTP synthase that catalyzes the formation of dCTP from dUTP, the final step in pyrimidine biosynthesis, whereas AAH1 is an adenine deaminase (adenine aminohydrolase), an enzyme of the purine salvage pathway, and converts adenosine to inosine     [33-36]  .	transcription
78998	1	335469	6	NULL	NULL	NULL	NULL	ATP	Chemical	depletion of	leads to					adenine nucleotides	Chemical	accumulation of			NULL	myocardial ischemia	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_17_10096_s_62	8626567	Effect of EHNA on the Adenine Nucleotide Pool in the  Postischemic HeartIt is well established that ATP depletion  during myocardial ischemia leads to accumulation of the diffusible  adenine nucleotides, adenosine and inosine, as well as the  nucleopurines, hypoxanthine and xanthine ( Fig. 1).	transcription
78999	2	335469	6	NULL	NULL	NULL	NULL	ATP	Chemical	depletion of	leads to					adenosine	Chemical	accumulation of 			NULL	myocardial ischemia	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_17_10096_s_62	8626567	Effect of EHNA on the Adenine Nucleotide Pool in the  Postischemic HeartIt is well established that ATP depletion  during myocardial ischemia leads to accumulation of the diffusible  adenine nucleotides, adenosine and inosine, as well as the  nucleopurines, hypoxanthine and xanthine ( Fig. 1).	transcription
79000	3	335469	6	NULL	NULL	NULL	NULL	ATP	Chemical	depletion of	leads to					inosine	Chemical	accumulation of 			NULL	myocardial ischemia	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_17_10096_s_62	8626567	Effect of EHNA on the Adenine Nucleotide Pool in the  Postischemic HeartIt is well established that ATP depletion  during myocardial ischemia leads to accumulation of the diffusible  adenine nucleotides, adenosine and inosine, as well as the  nucleopurines, hypoxanthine and xanthine ( Fig. 1).	transcription
79001	4	335469	6	NULL	NULL	0	NULL	ATP	Chemical	depletion of	leads to					hypoxanthine	Chemical	accumulation of 			NULL	myocardial ischemia	0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10096_s_62	8626567	Effect of EHNA on the Adenine Nucleotide Pool in the  Postischemic HeartIt is well established that ATP depletion  during myocardial ischemia leads to accumulation of the diffusible  adenine nucleotides, adenosine and inosine, as well as the  nucleopurines, hypoxanthine and xanthine ( Fig. 1).	transcription
79002	5	335469	6	NULL	NULL	0	NULL	ATP	Chemical	depletion of	leads to					xanthine	Chemical	accumulation of 			NULL	myocardial ischemia	0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10096_s_62	8626567	Effect of EHNA on the Adenine Nucleotide Pool in the  Postischemic HeartIt is well established that ATP depletion  during myocardial ischemia leads to accumulation of the diffusible  adenine nucleotides, adenosine and inosine, as well as the  nucleopurines, hypoxanthine and xanthine ( Fig. 1).	transcription
59068	1	335469	7	NULL	NULL	0	NULL	ATP		depletion of	leads to					adenine nucleotides		accumulation of;;diffusible 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_17_10096_s_62	8626567	Effect of EHNA on the Adenine Nucleotide Pool in the  Postischemic HeartIt is well established that ATP depletion  during myocardial ischemia leads to accumulation of the diffusible  adenine nucleotides, adenosine and inosine, as well as the  nucleopurines, hypoxanthine and xanthine ( Fig. 1).	transcription
59069	2	335469	7	NULL	NULL	0	NULL	statement 1			occur during					myocardial ischemia					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10096_s_62	8626567	Effect of EHNA on the Adenine Nucleotide Pool in the  Postischemic HeartIt is well established that ATP depletion  during myocardial ischemia leads to accumulation of the diffusible  adenine nucleotides, adenosine and inosine, as well as the  nucleopurines, hypoxanthine and xanthine ( Fig. 1).	transcription
59070	3	335469	7	NULL	NULL	0	NULL	ATP		depletion of	leads to					adenosine		accumulation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10096_s_62	8626567	Effect of EHNA on the Adenine Nucleotide Pool in the  Postischemic HeartIt is well established that ATP depletion  during myocardial ischemia leads to accumulation of the diffusible  adenine nucleotides, adenosine and inosine, as well as the  nucleopurines, hypoxanthine and xanthine ( Fig. 1).	transcription
59071	4	335469	7	NULL	NULL	0	NULL	statement 3			occur during					myocardial ischemia					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10096_s_62	8626567	Effect of EHNA on the Adenine Nucleotide Pool in the  Postischemic HeartIt is well established that ATP depletion  during myocardial ischemia leads to accumulation of the diffusible  adenine nucleotides, adenosine and inosine, as well as the  nucleopurines, hypoxanthine and xanthine ( Fig. 1).	transcription
59072	5	335469	7	NULL	NULL	0	NULL	ATP		depletion of	leads to					inosine		accumulation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10096_s_62	8626567	Effect of EHNA on the Adenine Nucleotide Pool in the  Postischemic HeartIt is well established that ATP depletion  during myocardial ischemia leads to accumulation of the diffusible  adenine nucleotides, adenosine and inosine, as well as the  nucleopurines, hypoxanthine and xanthine ( Fig. 1).	transcription
59073	6	335469	7	NULL	NULL	0	NULL	statement 5			occur during					myocardial ischemia					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10096_s_62	8626567	Effect of EHNA on the Adenine Nucleotide Pool in the  Postischemic HeartIt is well established that ATP depletion  during myocardial ischemia leads to accumulation of the diffusible  adenine nucleotides, adenosine and inosine, as well as the  nucleopurines, hypoxanthine and xanthine ( Fig. 1).	transcription
59074	7	335469	7	NULL	NULL	0	NULL	ATP		depletion of	leads to					hypoxanthine		accumulation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10096_s_62	8626567	Effect of EHNA on the Adenine Nucleotide Pool in the  Postischemic HeartIt is well established that ATP depletion  during myocardial ischemia leads to accumulation of the diffusible  adenine nucleotides, adenosine and inosine, as well as the  nucleopurines, hypoxanthine and xanthine ( Fig. 1).	transcription
59075	8	335469	7	NULL	NULL	0	NULL	statement 7			occur during					myocardial ischemia					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10096_s_62	8626567	Effect of EHNA on the Adenine Nucleotide Pool in the  Postischemic HeartIt is well established that ATP depletion  during myocardial ischemia leads to accumulation of the diffusible  adenine nucleotides, adenosine and inosine, as well as the  nucleopurines, hypoxanthine and xanthine ( Fig. 1).	transcription
59076	9	335469	7	NULL	NULL	0	NULL	ATP		depletion of	leads to					xanthine		accumulation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10096_s_62	8626567	Effect of EHNA on the Adenine Nucleotide Pool in the  Postischemic HeartIt is well established that ATP depletion  during myocardial ischemia leads to accumulation of the diffusible  adenine nucleotides, adenosine and inosine, as well as the  nucleopurines, hypoxanthine and xanthine ( Fig. 1).	transcription
59077	10	335469	7	NULL	NULL	0	NULL	statement 9			occur during					myocardial ischemia					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10096_s_62	8626567	Effect of EHNA on the Adenine Nucleotide Pool in the  Postischemic HeartIt is well established that ATP depletion  during myocardial ischemia leads to accumulation of the diffusible  adenine nucleotides, adenosine and inosine, as well as the  nucleopurines, hypoxanthine and xanthine ( Fig. 1).	transcription
59078	11	335469	7	NULL	NULL	0	NULL	hypoxanthine			is a type of					nucleopurine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10096_s_62	8626567	Effect of EHNA on the Adenine Nucleotide Pool in the  Postischemic HeartIt is well established that ATP depletion  during myocardial ischemia leads to accumulation of the diffusible  adenine nucleotides, adenosine and inosine, as well as the  nucleopurines, hypoxanthine and xanthine ( Fig. 1).	transcription
59079	12	335469	7	NULL	NULL	0	NULL	xanthine			is a type of					nucleopurine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10096_s_62	8626567	Effect of EHNA on the Adenine Nucleotide Pool in the  Postischemic HeartIt is well established that ATP depletion  during myocardial ischemia leads to accumulation of the diffusible  adenine nucleotides, adenosine and inosine, as well as the  nucleopurines, hypoxanthine and xanthine ( Fig. 1).	transcription
79003	1	335471	6	NULL	NULL	0	NULL	adenosine			is deaminated to					inosine					NULL	viral RNA	0	NULL	NULL	NULL	gw70_pnas_103_5_1440_s_168	16434471	Although expression of A3G is not stimulated by IFN in T cell line H9 ( ), one of the ISGs, adenine deaminase, catalyzes deamination of adenosine to inosine  in viral RNAs ( ).	transcription
79004	2	335471	6	NULL	NULL	0	NULL	IFN	GP		does not stimulate					A3G	GP	expression of			NULL	T cell line H9	0	NULL	NULL	NULL	gw70_pnas_103_5_1440_s_168	16434471	Although expression of A3G is not stimulated by IFN in T cell line H9 ( ), one of the ISGs, adenine deaminase, catalyzes deamination of adenosine to inosine  in viral RNAs ( ).	transcription
79005	3	335471	6	NULL	NULL	0	NULL	adenine deaminase	GP		catalyzes					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_103_5_1440_s_168	16434471	Although expression of A3G is not stimulated by IFN in T cell line H9 ( ), one of the ISGs, adenine deaminase, catalyzes deamination of adenosine to inosine  in viral RNAs ( ).	transcription
59098	1	335471	7	NULL	NULL	0	NULL	IFN 			does not stimulate					A3G		expression of			NULL	T cell line H9	0	NULL	NULL	NULL	gw70_pnas_103_5_1440_s_168	16434471	Although expression of A3G is not stimulated by IFN in T cell line H9 ( ), one of the ISGs, adenine deaminase, catalyzes deamination of adenosine to inosine  in viral RNAs ( ).	transcription
59099	2	335471	7	NULL	NULL	0	NULL	adenosine 			converted to					inosine					NULL	viral RNAs	0	NULL	NULL	NULL	gw70_pnas_103_5_1440_s_168	16434471	Although expression of A3G is not stimulated by IFN in T cell line H9 ( ), one of the ISGs, adenine deaminase, catalyzes deamination of adenosine to inosine  in viral RNAs ( ).	transcription
59100	3	335471	7	NULL	NULL	0	NULL	adenine deaminase			catalyze					statement 2		deamination of			NULL		0	NULL	NULL	NULL	gw70_pnas_103_5_1440_s_168	16434471	Although expression of A3G is not stimulated by IFN in T cell line H9 ( ), one of the ISGs, adenine deaminase, catalyzes deamination of adenosine to inosine  in viral RNAs ( ).	transcription
59101	4	335471	7	NULL	NULL	0	NULL	adenine deaminase			is a type of					ISGs					NULL		0	NULL	NULL	NULL	gw70_pnas_103_5_1440_s_168	16434471	Although expression of A3G is not stimulated by IFN in T cell line H9 ( ), one of the ISGs, adenine deaminase, catalyzes deamination of adenosine to inosine  in viral RNAs ( ).	transcription
59102	1	335472	7	NULL	NULL	0	NULL	hypoxanthine			incorporated into					cell lines					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_31_19488_s_150	9235951	100 muM concentrations of either hypoxanthine, adenine, adenosine, inosine, or guanine inhibited the incorporation of 1.8 muM [14]hypoxanthine into all cell lines tested by 80-90%.	transcription
59103	2	335472	7	NULL	NULL	0	NULL	hypoxanthine			inhibit					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_31_19488_s_150	9235951	100 muM concentrations of either hypoxanthine, adenine, adenosine, inosine, or guanine inhibited the incorporation of 1.8 muM [14]hypoxanthine into all cell lines tested by 80-90%.	transcription
59104	3	335472	7	NULL	NULL	0	NULL	adenine			inhibit					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_31_19488_s_150	9235951	100 muM concentrations of either hypoxanthine, adenine, adenosine, inosine, or guanine inhibited the incorporation of 1.8 muM [14]hypoxanthine into all cell lines tested by 80-90%.	transcription
59105	4	335472	7	NULL	NULL	0	NULL	adenosine 			inhibit					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_31_19488_s_150	9235951	100 muM concentrations of either hypoxanthine, adenine, adenosine, inosine, or guanine inhibited the incorporation of 1.8 muM [14]hypoxanthine into all cell lines tested by 80-90%.	transcription
59106	5	335472	7	NULL	NULL	0	NULL	inosine			inhibit					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_31_19488_s_150	9235951	100 muM concentrations of either hypoxanthine, adenine, adenosine, inosine, or guanine inhibited the incorporation of 1.8 muM [14]hypoxanthine into all cell lines tested by 80-90%.	transcription
59107	6	335472	7	NULL	NULL	0	NULL	guanine			inhibit					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_31_19488_s_150	9235951	100 muM concentrations of either hypoxanthine, adenine, adenosine, inosine, or guanine inhibited the incorporation of 1.8 muM [14]hypoxanthine into all cell lines tested by 80-90%.	transcription
79006	1	335473	6	NULL	NULL	0	NULL	EHNA	Chemical		is					Erythro-9-(2-hydroxy-3-nonyl)adenine	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_mol-cell-biochem_281_1-2_16328964_s_8	16328964	Erythro-9-(2-hydroxy-3-nonyl)adenine (EHNA),  an adenosine deaminase inhibitor, abolished the TNF-alpha induced inosine  increase, nitrite accumulation and nitric oxide synthase activity.	transcription
79007	2	335473	6	NULL	NULL	0	NULL	EHNA	Chemical		is a type of					adenosine deaminase inhibitor	GP				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_mol-cell-biochem_281_1-2_16328964_s_8	16328964	Erythro-9-(2-hydroxy-3-nonyl)adenine (EHNA),  an adenosine deaminase inhibitor, abolished the TNF-alpha induced inosine  increase, nitrite accumulation and nitric oxide synthase activity.	transcription
79008	3	335473	6	NULL	NULL	0	NULL	TNF-alpha	GP		induces					inosine	Chemical	increase of 			NULL		0	NULL	NULL	NULL	abs-batch0540-0549_mol-cell-biochem_281_1-2_16328964_s_8	16328964	Erythro-9-(2-hydroxy-3-nonyl)adenine (EHNA),  an adenosine deaminase inhibitor, abolished the TNF-alpha induced inosine  increase, nitrite accumulation and nitric oxide synthase activity.	transcription
79009	4	335473	6	NULL	NULL	0	NULL	TNF-alpha	GP		induces					nitrite	Chemical	accumulation of 			NULL		0	NULL	NULL	NULL	abs-batch0540-0549_mol-cell-biochem_281_1-2_16328964_s_8	16328964	Erythro-9-(2-hydroxy-3-nonyl)adenine (EHNA),  an adenosine deaminase inhibitor, abolished the TNF-alpha induced inosine  increase, nitrite accumulation and nitric oxide synthase activity.	transcription
79010	5	335473	6	NULL	NULL	0	NULL	TNF-alpha	GP		induces					nitric oxide synthase activity	Process				NULL		0	NULL	NULL	NULL	abs-batch0540-0549_mol-cell-biochem_281_1-2_16328964_s_8	16328964	Erythro-9-(2-hydroxy-3-nonyl)adenine (EHNA),  an adenosine deaminase inhibitor, abolished the TNF-alpha induced inosine  increase, nitrite accumulation and nitric oxide synthase activity.	transcription
59108	1	335473	7	NULL	NULL	0	NULL	TNF-alpha			induce					inosine		increase in			NULL		0	NULL	NULL	NULL	abs-batch0540-0549_mol-cell-biochem_281_1-2_16328964_s_8	16328964	Erythro-9-(2-hydroxy-3-nonyl)adenine (EHNA),  an adenosine deaminase inhibitor, abolished the TNF-alpha induced inosine  increase, nitrite accumulation and nitric oxide synthase activity.	transcription
59109	2	335473	7	NULL	NULL	0	NULL	TNF-alpha			induce					nitrite		accumulation of			NULL		0	NULL	NULL	NULL	abs-batch0540-0549_mol-cell-biochem_281_1-2_16328964_s_8	16328964	Erythro-9-(2-hydroxy-3-nonyl)adenine (EHNA),  an adenosine deaminase inhibitor, abolished the TNF-alpha induced inosine  increase, nitrite accumulation and nitric oxide synthase activity.	transcription
59110	3	335473	7	NULL	NULL	0	NULL	TNF-alpha			induce					nitric oxide synthase		activity of			NULL		0	NULL	NULL	NULL	abs-batch0540-0549_mol-cell-biochem_281_1-2_16328964_s_8	16328964	Erythro-9-(2-hydroxy-3-nonyl)adenine (EHNA),  an adenosine deaminase inhibitor, abolished the TNF-alpha induced inosine  increase, nitrite accumulation and nitric oxide synthase activity.	transcription
59111	4	335473	7	NULL	NULL	0	NULL	EHNA			abolish					statement 1					NULL		0	NULL	NULL	NULL	abs-batch0540-0549_mol-cell-biochem_281_1-2_16328964_s_8	16328964	Erythro-9-(2-hydroxy-3-nonyl)adenine (EHNA),  an adenosine deaminase inhibitor, abolished the TNF-alpha induced inosine  increase, nitrite accumulation and nitric oxide synthase activity.	transcription
59112	5	335473	7	NULL	NULL	0	NULL	EHNA			abolish					statement 2					NULL		0	NULL	NULL	NULL	abs-batch0540-0549_mol-cell-biochem_281_1-2_16328964_s_8	16328964	Erythro-9-(2-hydroxy-3-nonyl)adenine (EHNA),  an adenosine deaminase inhibitor, abolished the TNF-alpha induced inosine  increase, nitrite accumulation and nitric oxide synthase activity.	transcription
59113	6	335473	7	NULL	NULL	0	NULL	EHNA			abolish					statement 3					NULL		0	NULL	NULL	NULL	abs-batch0540-0549_mol-cell-biochem_281_1-2_16328964_s_8	16328964	Erythro-9-(2-hydroxy-3-nonyl)adenine (EHNA),  an adenosine deaminase inhibitor, abolished the TNF-alpha induced inosine  increase, nitrite accumulation and nitric oxide synthase activity.	transcription
59114	7	335473	7	NULL	NULL	0	NULL	EHNA			is					Erythro-9-(2-hydroxy-3-nonyl)adenine					NULL		0	NULL	NULL	NULL	abs-batch0540-0549_mol-cell-biochem_281_1-2_16328964_s_8	16328964	Erythro-9-(2-hydroxy-3-nonyl)adenine (EHNA),  an adenosine deaminase inhibitor, abolished the TNF-alpha induced inosine  increase, nitrite accumulation and nitric oxide synthase activity.	transcription
59116	8	335473	7	NULL	NULL	0	NULL	EHNA			is a type of					adenosine deaminase inhibitor					NULL		0	NULL	NULL	NULL	abs-batch0540-0549_mol-cell-biochem_281_1-2_16328964_s_8	16328964	Erythro-9-(2-hydroxy-3-nonyl)adenine (EHNA),  an adenosine deaminase inhibitor, abolished the TNF-alpha induced inosine  increase, nitrite accumulation and nitric oxide synthase activity.	transcription
59117	1	335474	7	NULL	NULL	0	NULL	T. b. brucei			salvage					adenosine					NULL		0	NULL	NULL	NULL	gw60_microbesinfect_3_9_763_s_151	11489425	T. b. brucei were reported to salvage adenosine via the transporters, P1, which is specific for adenosine and inosine, and P2, which mediates transport of adenosine, adenine, melanophenyl arsenicals and diamidines  38;   51 and   52.	transcription
59118	2	335474	7	NULL	NULL	0	NULL	statement 1			via					P1 transporter					NULL		0	NULL	NULL	NULL	gw60_microbesinfect_3_9_763_s_151	11489425	T. b. brucei were reported to salvage adenosine via the transporters, P1, which is specific for adenosine and inosine, and P2, which mediates transport of adenosine, adenine, melanophenyl arsenicals and diamidines  38;   51 and   52.	transcription
59119	3	335474	7	NULL	NULL	0	NULL	P1 transporter			is specific for					adenosine					NULL		0	NULL	NULL	NULL	gw60_microbesinfect_3_9_763_s_151	11489425	T. b. brucei were reported to salvage adenosine via the transporters, P1, which is specific for adenosine and inosine, and P2, which mediates transport of adenosine, adenine, melanophenyl arsenicals and diamidines  38;   51 and   52.	transcription
59120	4	335474	7	NULL	NULL	0	NULL	P1 transporter			is specific for					inosine					NULL		NULL	NULL	NULL	NULL	gw60_microbesinfect_3_9_763_s_151	11489425	T. b. brucei were reported to salvage adenosine via the transporters, P1, which is specific for adenosine and inosine, and P2, which mediates transport of adenosine, adenine, melanophenyl arsenicals and diamidines  38;   51 and   52.	transcription
59124	5	335474	7	NULL	NULL	0	NULL	P2			mediates					adenosine		transport of			NULL		0	NULL	NULL	NULL	gw60_microbesinfect_3_9_763_s_151	11489425	T. b. brucei were reported to salvage adenosine via the transporters, P1, which is specific for adenosine and inosine, and P2, which mediates transport of adenosine, adenine, melanophenyl arsenicals and diamidines  38;   51 and   52.	transcription
59129	6	335474	7	NULL	NULL	0	NULL	P2			mediates					adenine		transport of			NULL		0	NULL	NULL	NULL	gw60_microbesinfect_3_9_763_s_151	11489425	T. b. brucei were reported to salvage adenosine via the transporters, P1, which is specific for adenosine and inosine, and P2, which mediates transport of adenosine, adenine, melanophenyl arsenicals and diamidines  38;   51 and   52.	transcription
59134	7	335474	7	NULL	NULL	0	NULL	P2			mediates					melanophenyl arsenicals		transport of			NULL		NULL	NULL	NULL	NULL	gw60_microbesinfect_3_9_763_s_151	11489425	T. b. brucei were reported to salvage adenosine via the transporters, P1, which is specific for adenosine and inosine, and P2, which mediates transport of adenosine, adenine, melanophenyl arsenicals and diamidines  38;   51 and   52.	transcription
59138	8	335474	7	NULL	NULL	0	NULL	P2			mediates					diamidines		transport of			NULL		0	NULL	NULL	NULL	gw60_microbesinfect_3_9_763_s_151	11489425	T. b. brucei were reported to salvage adenosine via the transporters, P1, which is specific for adenosine and inosine, and P2, which mediates transport of adenosine, adenine, melanophenyl arsenicals and diamidines  38;   51 and   52.	transcription
79011	1	335475	6	NULL	NULL	0	NULL	adenosine	Chemical		is formed from					adenine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_3_457_s_230	9457844	The enzyme activities present in both halobacteria suggest that this conversion implies formation of adenosine from adenine and ribose-1-phosphate catalyzed by adenosine phosphorylase, followed by deamination of adenosine to inosine catalyzed by adenosine deaminase.	transcription
79012	2	335475	6	NULL	NULL	0	NULL	adenosine	Chemical		is formed from					ribose-1-phosphate	GP				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_3_457_s_230	9457844	The enzyme activities present in both halobacteria suggest that this conversion implies formation of adenosine from adenine and ribose-1-phosphate catalyzed by adenosine phosphorylase, followed by deamination of adenosine to inosine catalyzed by adenosine deaminase.	transcription
79013	3	335475	6	NULL	NULL	0	NULL	statement 1	Process		occurs simultaneously with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_3_457_s_230	9457844	The enzyme activities present in both halobacteria suggest that this conversion implies formation of adenosine from adenine and ribose-1-phosphate catalyzed by adenosine phosphorylase, followed by deamination of adenosine to inosine catalyzed by adenosine deaminase.	transcription
79014	4	335475	6	NULL	NULL	0	NULL	adenosine phosphorylase	GP		catalyzes					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_3_457_s_230	9457844	The enzyme activities present in both halobacteria suggest that this conversion implies formation of adenosine from adenine and ribose-1-phosphate catalyzed by adenosine phosphorylase, followed by deamination of adenosine to inosine catalyzed by adenosine deaminase.	transcription
79015	5	335475	6	NULL	NULL	0	NULL	adenosine	Chemical		is deaminated to					inosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_3_457_s_230	9457844	The enzyme activities present in both halobacteria suggest that this conversion implies formation of adenosine from adenine and ribose-1-phosphate catalyzed by adenosine phosphorylase, followed by deamination of adenosine to inosine catalyzed by adenosine deaminase.	transcription
79016	6	335475	6	NULL	NULL	0	NULL	statement 5	Process		is catalyzed by					adenosine deaminase	GP				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_3_457_s_230	9457844	The enzyme activities present in both halobacteria suggest that this conversion implies formation of adenosine from adenine and ribose-1-phosphate catalyzed by adenosine phosphorylase, followed by deamination of adenosine to inosine catalyzed by adenosine deaminase.	transcription
59143	1	335475	7	NULL	NULL	0	NULL	adenosine			formed from					adenine					NULL	halobacteria	NULL	NULL	NULL	NULL	gw60_jbacteriol_180_3_457_s_230	9457844	The enzyme activities present in both halobacteria suggest that this conversion implies formation of adenosine from adenine and ribose-1-phosphate catalyzed by adenosine phosphorylase, followed by deamination of adenosine to inosine catalyzed by adenosine deaminase.	transcription
59145	2	335475	7	NULL	NULL	0	NULL	adenosine			formed from					ribose-1-phosphate					NULL	halobacteria	NULL	NULL	NULL	NULL	gw60_jbacteriol_180_3_457_s_230	9457844	The enzyme activities present in both halobacteria suggest that this conversion implies formation of adenosine from adenine and ribose-1-phosphate catalyzed by adenosine phosphorylase, followed by deamination of adenosine to inosine catalyzed by adenosine deaminase.	transcription
59146	3	335475	7	NULL	NULL	0	NULL	statement 1			occur simulataneous with					statement 2					NULL	halobacteria	NULL	NULL	NULL	NULL	gw60_jbacteriol_180_3_457_s_230	9457844	The enzyme activities present in both halobacteria suggest that this conversion implies formation of adenosine from adenine and ribose-1-phosphate catalyzed by adenosine phosphorylase, followed by deamination of adenosine to inosine catalyzed by adenosine deaminase.	transcription
59174	4	335475	7	NULL	NULL	0	NULL	adenosine phosphorylase			catalyze					statement 3					NULL	halobacteria	NULL	NULL	NULL	NULL	gw60_jbacteriol_180_3_457_s_230	9457844	The enzyme activities present in both halobacteria suggest that this conversion implies formation of adenosine from adenine and ribose-1-phosphate catalyzed by adenosine phosphorylase, followed by deamination of adenosine to inosine catalyzed by adenosine deaminase.	transcription
59175	5	335475	7	NULL	NULL	0	NULL	adenosine			deaminates to					inosine					NULL	halobacteria	NULL	NULL	NULL	NULL	gw60_jbacteriol_180_3_457_s_230	9457844	The enzyme activities present in both halobacteria suggest that this conversion implies formation of adenosine from adenine and ribose-1-phosphate catalyzed by adenosine phosphorylase, followed by deamination of adenosine to inosine catalyzed by adenosine deaminase.	transcription
59176	6	335475	7	NULL	NULL	0	NULL	adenosine deaminase			catalyze					statement 5					NULL	halobacteria	NULL	NULL	NULL	NULL	gw60_jbacteriol_180_3_457_s_230	9457844	The enzyme activities present in both halobacteria suggest that this conversion implies formation of adenosine from adenine and ribose-1-phosphate catalyzed by adenosine phosphorylase, followed by deamination of adenosine to inosine catalyzed by adenosine deaminase.	transcription
59177	7	335475	7	NULL	NULL	0	NULL	statement 5			is followed by					statement 4					NULL	halobacteria	NULL	NULL	NULL	NULL	gw60_jbacteriol_180_3_457_s_230	9457844	The enzyme activities present in both halobacteria suggest that this conversion implies formation of adenosine from adenine and ribose-1-phosphate catalyzed by adenosine phosphorylase, followed by deamination of adenosine to inosine catalyzed by adenosine deaminase.	transcription
79017	1	335476	6	NULL	NULL	0	NULL	IMP	Chemical		is oxidized to					XMP	Chemical				NULL		0	NULL	NULL	NULL	gw60_cell_85_6_921_s_10	8681386	IMPDH catalyzes the nicotinamide adenine dinucleotide (NAD)-dependent oxidation of inosine-5''-monophosphate  (IMP) to xanthosine-5''-monophosphate (XMP), which is the committed step in de novo guanosine nucleotide  biosynthesis (Crabtree and Henderson, 1971   ;  Snyder et al., 1972   ;  Jackson  et al., 1975   ;  Weber, 1983   ).	transcription
79018	2	335476	6	NULL	NULL	0	NULL	IMPDH	GP		catalyzes					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_cell_85_6_921_s_10	8681386	IMPDH catalyzes the nicotinamide adenine dinucleotide (NAD)-dependent oxidation of inosine-5''-monophosphate  (IMP) to xanthosine-5''-monophosphate (XMP), which is the committed step in de novo guanosine nucleotide  biosynthesis (Crabtree and Henderson, 1971   ;  Snyder et al., 1972   ;  Jackson  et al., 1975   ;  Weber, 1983   ).	transcription
79019	3	335476	6	NULL	NULL	0	NULL	statement 1	Process		is dependent on					NAD	Chemical				NULL		0	NULL	NULL	NULL	gw60_cell_85_6_921_s_10	8681386	IMPDH catalyzes the nicotinamide adenine dinucleotide (NAD)-dependent oxidation of inosine-5''-monophosphate  (IMP) to xanthosine-5''-monophosphate (XMP), which is the committed step in de novo guanosine nucleotide  biosynthesis (Crabtree and Henderson, 1971   ;  Snyder et al., 1972   ;  Jackson  et al., 1975   ;  Weber, 1983   ).	transcription
79020	4	335476	6	NULL	NULL	0	NULL	NAD	Chemical		is					nicotinamide adenine dinucleotide	Chemical				NULL		0	NULL	NULL	NULL	gw60_cell_85_6_921_s_10	8681386	IMPDH catalyzes the nicotinamide adenine dinucleotide (NAD)-dependent oxidation of inosine-5''-monophosphate  (IMP) to xanthosine-5''-monophosphate (XMP), which is the committed step in de novo guanosine nucleotide  biosynthesis (Crabtree and Henderson, 1971   ;  Snyder et al., 1972   ;  Jackson  et al., 1975   ;  Weber, 1983   ).	transcription
79021	5	335476	6	NULL	NULL	0	NULL	IMP	Chemical		is					inosine-5''-monophosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_cell_85_6_921_s_10	8681386	IMPDH catalyzes the nicotinamide adenine dinucleotide (NAD)-dependent oxidation of inosine-5''-monophosphate  (IMP) to xanthosine-5''-monophosphate (XMP), which is the committed step in de novo guanosine nucleotide  biosynthesis (Crabtree and Henderson, 1971   ;  Snyder et al., 1972   ;  Jackson  et al., 1975   ;  Weber, 1983   ).	transcription
79022	6	335476	6	NULL	NULL	0	NULL	XMP	Chemical		is					xanthosine-5''-monophosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_cell_85_6_921_s_10	8681386	IMPDH catalyzes the nicotinamide adenine dinucleotide (NAD)-dependent oxidation of inosine-5''-monophosphate  (IMP) to xanthosine-5''-monophosphate (XMP), which is the committed step in de novo guanosine nucleotide  biosynthesis (Crabtree and Henderson, 1971   ;  Snyder et al., 1972   ;  Jackson  et al., 1975   ;  Weber, 1983   ).	transcription
59178	1	335476	7	NULL	NULL	0	NULL	IMP			oxidizes to					XMP					NULL		0	NULL	NULL	NULL	gw60_cell_85_6_921_s_10	8681386	IMPDH catalyzes the nicotinamide adenine dinucleotide (NAD)-dependent oxidation of inosine-5''-monophosphate  (IMP) to xanthosine-5''-monophosphate (XMP), which is the committed step in de novo guanosine nucleotide  biosynthesis (Crabtree and Henderson, 1971   ;  Snyder et al., 1972   ;  Jackson  et al., 1975   ;  Weber, 1983   ).	transcription
59179	2	335476	7	NULL	NULL	0	NULL	statement 1			depends on					NAD					NULL		0	NULL	NULL	NULL	gw60_cell_85_6_921_s_10	8681386	IMPDH catalyzes the nicotinamide adenine dinucleotide (NAD)-dependent oxidation of inosine-5''-monophosphate  (IMP) to xanthosine-5''-monophosphate (XMP), which is the committed step in de novo guanosine nucleotide  biosynthesis (Crabtree and Henderson, 1971   ;  Snyder et al., 1972   ;  Jackson  et al., 1975   ;  Weber, 1983   ).	transcription
59180	3	335476	7	NULL	NULL	0	NULL	IMPDH			catalyzes					statement 2					NULL		0	NULL	NULL	NULL	gw60_cell_85_6_921_s_10	8681386	IMPDH catalyzes the nicotinamide adenine dinucleotide (NAD)-dependent oxidation of inosine-5''-monophosphate  (IMP) to xanthosine-5''-monophosphate (XMP), which is the committed step in de novo guanosine nucleotide  biosynthesis (Crabtree and Henderson, 1971   ;  Snyder et al., 1972   ;  Jackson  et al., 1975   ;  Weber, 1983   ).	transcription
59181	4	335476	7	NULL	NULL	0	NULL	statement 1			committed step in					de novo guanosine nucleotide biosynthesis					NULL		0	NULL	NULL	NULL	gw60_cell_85_6_921_s_10	8681386	IMPDH catalyzes the nicotinamide adenine dinucleotide (NAD)-dependent oxidation of inosine-5''-monophosphate  (IMP) to xanthosine-5''-monophosphate (XMP), which is the committed step in de novo guanosine nucleotide  biosynthesis (Crabtree and Henderson, 1971   ;  Snyder et al., 1972   ;  Jackson  et al., 1975   ;  Weber, 1983   ).	transcription
59182	5	335476	7	NULL	NULL	0	NULL	NAD			is					nicotinamide adenine dinucleotide					NULL		0	NULL	NULL	NULL	gw60_cell_85_6_921_s_10	8681386	IMPDH catalyzes the nicotinamide adenine dinucleotide (NAD)-dependent oxidation of inosine-5''-monophosphate  (IMP) to xanthosine-5''-monophosphate (XMP), which is the committed step in de novo guanosine nucleotide  biosynthesis (Crabtree and Henderson, 1971   ;  Snyder et al., 1972   ;  Jackson  et al., 1975   ;  Weber, 1983   ).	transcription
59183	6	335476	7	NULL	NULL	0	NULL	IMP			is					inosine-5''-monophosphate					NULL		0	NULL	NULL	NULL	gw60_cell_85_6_921_s_10	8681386	IMPDH catalyzes the nicotinamide adenine dinucleotide (NAD)-dependent oxidation of inosine-5''-monophosphate  (IMP) to xanthosine-5''-monophosphate (XMP), which is the committed step in de novo guanosine nucleotide  biosynthesis (Crabtree and Henderson, 1971   ;  Snyder et al., 1972   ;  Jackson  et al., 1975   ;  Weber, 1983   ).	transcription
59184	7	335476	7	NULL	NULL	0	NULL	XMP			is					xanthosine-5''-monophosphate					NULL		0	NULL	NULL	NULL	gw60_cell_85_6_921_s_10	8681386	IMPDH catalyzes the nicotinamide adenine dinucleotide (NAD)-dependent oxidation of inosine-5''-monophosphate  (IMP) to xanthosine-5''-monophosphate (XMP), which is the committed step in de novo guanosine nucleotide  biosynthesis (Crabtree and Henderson, 1971   ;  Snyder et al., 1972   ;  Jackson  et al., 1975   ;  Weber, 1983   ).	transcription
59185	1	335479	7	NULL	NULL	0	NULL	P1 type system 			mediates					adenosine		uptake of			NULL	BF life cycle stage	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_24_21499_s_14	11937511	The P1 type system mediates the uptake of purine nucleosides (adenosine, inosine, and guanosine) and is detected in both BF and PF life cycle stages, and the P2 type system mediates the uptake of adenosine and adenine, as well as several anti-trypanosomal drugs, and is detected only in the BF ( 6,  7) parasites.	transcription
59186	2	335479	7	NULL	NULL	0	NULL	P1 type system 			mediates					inosine		uptake of			NULL	BF life cycle stage	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_24_21499_s_14	11937511	The P1 type system mediates the uptake of purine nucleosides (adenosine, inosine, and guanosine) and is detected in both BF and PF life cycle stages, and the P2 type system mediates the uptake of adenosine and adenine, as well as several anti-trypanosomal drugs, and is detected only in the BF ( 6,  7) parasites.	transcription
59187	3	335479	7	NULL	NULL	0	NULL	P1 type system 			mediates					guanosine		uptake of			NULL	BF life cycle stage	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_24_21499_s_14	11937511	The P1 type system mediates the uptake of purine nucleosides (adenosine, inosine, and guanosine) and is detected in both BF and PF life cycle stages, and the P2 type system mediates the uptake of adenosine and adenine, as well as several anti-trypanosomal drugs, and is detected only in the BF ( 6,  7) parasites.	transcription
59188	4	335479	7	NULL	NULL	0	NULL	adenosine 			is a type of					purine nucleoside					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_24_21499_s_14	11937511	The P1 type system mediates the uptake of purine nucleosides (adenosine, inosine, and guanosine) and is detected in both BF and PF life cycle stages, and the P2 type system mediates the uptake of adenosine and adenine, as well as several anti-trypanosomal drugs, and is detected only in the BF ( 6,  7) parasites.	transcription
59189	5	335479	7	NULL	NULL	0	NULL	inosine			is a type of					purine nucleoside					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_24_21499_s_14	11937511	The P1 type system mediates the uptake of purine nucleosides (adenosine, inosine, and guanosine) and is detected in both BF and PF life cycle stages, and the P2 type system mediates the uptake of adenosine and adenine, as well as several anti-trypanosomal drugs, and is detected only in the BF ( 6,  7) parasites.	transcription
59190	6	335479	7	NULL	NULL	0	NULL	guanosine			is a type of					purine nucleoside					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_24_21499_s_14	11937511	The P1 type system mediates the uptake of purine nucleosides (adenosine, inosine, and guanosine) and is detected in both BF and PF life cycle stages, and the P2 type system mediates the uptake of adenosine and adenine, as well as several anti-trypanosomal drugs, and is detected only in the BF ( 6,  7) parasites.	transcription
59191	7	335479	7	NULL	NULL	0	NULL	P1 type system 			mediates					adenosine		uptake of			NULL	PF life cycle stage	0	NULL	NULL	NULL	gw60_jbiolchem_277_24_21499_s_14	11937511	The P1 type system mediates the uptake of purine nucleosides (adenosine, inosine, and guanosine) and is detected in both BF and PF life cycle stages, and the P2 type system mediates the uptake of adenosine and adenine, as well as several anti-trypanosomal drugs, and is detected only in the BF ( 6,  7) parasites.	transcription
59192	8	335479	7	NULL	NULL	0	NULL	P1 type system 			mediate					inosine		uptake of			NULL	PF life cycle stage	0	NULL	NULL	NULL	gw60_jbiolchem_277_24_21499_s_14	11937511	The P1 type system mediates the uptake of purine nucleosides (adenosine, inosine, and guanosine) and is detected in both BF and PF life cycle stages, and the P2 type system mediates the uptake of adenosine and adenine, as well as several anti-trypanosomal drugs, and is detected only in the BF ( 6,  7) parasites.	transcription
59193	9	335479	7	NULL	NULL	0	NULL	P1 type system 			mediates					guanosine		uptake of			NULL	PF life cycle stage	0	NULL	NULL	NULL	gw60_jbiolchem_277_24_21499_s_14	11937511	The P1 type system mediates the uptake of purine nucleosides (adenosine, inosine, and guanosine) and is detected in both BF and PF life cycle stages, and the P2 type system mediates the uptake of adenosine and adenine, as well as several anti-trypanosomal drugs, and is detected only in the BF ( 6,  7) parasites.	transcription
59194	10	335479	7	NULL	NULL	0	NULL	P2 type system			mediates					adenosine		uptake of			NULL	BF parasites	0	NULL	NULL	NULL	gw60_jbiolchem_277_24_21499_s_14	11937511	The P1 type system mediates the uptake of purine nucleosides (adenosine, inosine, and guanosine) and is detected in both BF and PF life cycle stages, and the P2 type system mediates the uptake of adenosine and adenine, as well as several anti-trypanosomal drugs, and is detected only in the BF ( 6,  7) parasites.	transcription
59195	11	335479	7	NULL	NULL	0	NULL	P2 type system			mediates					adenine		uptake of			NULL	BF parasites	0	NULL	NULL	NULL	gw60_jbiolchem_277_24_21499_s_14	11937511	The P1 type system mediates the uptake of purine nucleosides (adenosine, inosine, and guanosine) and is detected in both BF and PF life cycle stages, and the P2 type system mediates the uptake of adenosine and adenine, as well as several anti-trypanosomal drugs, and is detected only in the BF ( 6,  7) parasites.	transcription
59196	12	335479	7	NULL	NULL	0	NULL	P2 type system			mediates					anti-trypanosomal drugs		uptake of			NULL	BF parasites	0	NULL	NULL	NULL	gw60_jbiolchem_277_24_21499_s_14	11937511	The P1 type system mediates the uptake of purine nucleosides (adenosine, inosine, and guanosine) and is detected in both BF and PF life cycle stages, and the P2 type system mediates the uptake of adenosine and adenine, as well as several anti-trypanosomal drugs, and is detected only in the BF ( 6,  7) parasites.	transcription
79097	1	335481	6	NULL	NULL	0	NULL	astrocytes	Cell		release					adenine nucleotides	Chemical				NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
79098	2	335481	6	NULL	NULL	0	NULL	astrocytes	Chemical		release					adenosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
79099	3	335481	6	NULL	NULL	0	NULL	neurons	CellComponent		release					purines	Chemical				NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
79100	4	335481	6	NULL	NULL	0	NULL	statement 3	Process		occurs during					glycolysis	Process	inhibition of			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
79101	5	335481	6	NULL	NULL	0	NULL	statement 3	Process		occurs during					oxidative phosphorylation	Process	inhibition of			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59200	1	335481	7	NULL	NULL	0	NULL	astrocytes			release					adenine nucleotides					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59201	2	335481	7	NULL	NULL	0	NULL	astrocytes			release					adenosine					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59202	3	335481	7	NULL	NULL	0	NULL	neurons			release					adenine nucleotides					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59203	4	335481	7	NULL	NULL	0	NULL	neurons			release					adenosine					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59204	5	335481	7	NULL	NULL	0	NULL	statement 1			more significantly than					statement 3					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59205	6	335481	7	NULL	NULL	0	NULL	statement 2			more significantly than					statement 4					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59206	7	335481	7	NULL	NULL	0	NULL	neurons			release					purines					NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59207	8	335481	7	NULL	NULL	0	NULL	statement 7			during					glycolysis		inhibition of			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59208	9	335481	7	NULL	NULL	0	NULL	statement 7			during					oxidative phosphorylation 		inhibition of			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59209	10	335481	7	NULL	NULL	0	NULL	statement 8		release from	is greater than					statement 9		release from			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59210	11	335481	7	NULL	NULL	0	NULL	astrocytes			release					purines					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59211	12	335481	7	NULL	NULL	0	NULL	statement 11			during					glycolysis		inhibition of			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59212	13	335481	7	NULL	NULL	0	NULL	statement 11			during					oxidative phosphorylation 		inhibition of			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59213	14	335481	7	NULL	NULL	0	NULL	statement 12		release from	is same as					statement 13		release from			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59214	15	335481	7	NULL	NULL	0	NULL	neurons			release					inosine					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59285	16	335481	7	NULL	NULL	0	NULL	neurons			release					hypoxanthine					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59286	17	335481	7	NULL	NULL	0	NULL	NaCN			induce					statement 15					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59287	18	335481	7	NULL	NULL	0	NULL	NACN			induce					statement 16					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59288	19	335481	7	NULL	NULL	0	NULL	IAA			induce					statement 15					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59289	20	335481	7	NULL	NULL	0	NULL	IAA			induce					statement 16					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59290	21	335481	7	NULL	NULL	0	NULL	statement 17		release from	is same as					statement 19		release from			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59291	22	335481	7	NULL	NULL	0	NULL	statement 18		release from	is same as					statement 20		release from			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59292	23	335481	7	NULL	NULL	0	NULL	astrocytes			release					hypoxanthine					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59293	24	335481	7	NULL	NULL	0	NULL	astrocytes			release					inosine					NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59294	25	335481	7	NULL	NULL	0	NULL	NACN			induce					statement 23					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59295	26	335481	7	NULL	NULL	0	NULL	IAA			induce					statement 23					NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59296	27	335481	7	NULL	NULL	0	NULL	NACN			induce					statement 24					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59297	28	335481	7	NULL	NULL	0	NULL	IAA			induce					statement 24					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59298	29	335481	7	NULL	NULL	0	NULL	statement 25		release from	is greater than					statement 18		release from			NULL		NULL	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59299	30	335481	7	NULL	NULL	0	NULL	statement 28		release from	is greater than					statement 20		release from			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59300	31	335481	7	NULL	NULL	0	NULL	statement 27		release from	is greater than					statement 17		release from			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59301	32	335481	7	NULL	NULL	0	NULL	statement 26		release from	is greater than					statement 19		release from			NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59302	33	335481	7	NULL	NULL	0	NULL	OGD			increase		significantly			statement 4					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59303	34	335481	7	NULL	NULL	0	NULL	NaCN 			increase		significantly			statement 4					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59304	35	335481	7	NULL	NULL	0	NULL	 IAA			increase		significantly			statement 4					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59305	36	335481	7	NULL	NULL	0	NULL	OGD			does not increase					statement 2					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59306	37	335481	7	NULL	NULL	0	NULL	NACN			does not increase					statement 2					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59307	38	335481	7	NULL	NULL	0	NULL	IAA			does not increase					statement 2					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59308	39	335481	7	NULL	NULL	0	NULL	DPR			blocks					statement 15					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59309	40	335481	7	NULL	NULL	0	NULL	DPR			blocks					statement 24					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59310	41	335481	7	NULL	NULL	0	NULL	DPR			blocks					statement 4					NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_43_5_836_s_216	12384169	The primary findings of this study are that (a) astrocytes released significantly more [3]adenine nucleotides and [3]adenosine than neurons, (b) neurons released greater amounts of [3]purines during inhibition of glycolysis compared to inhibition of oxidative phosphorylation while astrocytes released similar amounts with both stimuli, (c) NaCN and IAA treatments induced the release of similar amounts of [3]inosine and [3]hypoxanthine from neurons and ~2-4 fold more [3]hypoxanthine than [3]inosine from astrocytes, (d) OGD, NaCN and IAA conditions produced significant increases in [3]adenosine release from neurons but not astrocytes, and (e) DPR blocked [3]inosine release from both astrocytes and neurons but only blocked [3]adenosine release from neurons.	transcription
59311	1	335483	7	NULL	NULL	0	NULL	P1			mediates					adenosine		uptake of			NULL	T. b. brucei bloodstream	NULL	NULL	NULL	NULL	gw60_molpharmacol_56_6_1162_s_102	10570043	View this table:   [in this window]   [in a new window]     [[ TABLE 1        Ki ]] values for potential inhibitors of P1- and P2-mediated adenosine uptake in  T. b. brucei bloodstream forms    Initial rates of transport were measured by incubating 107 cells for 10 s with [3]adenosine in the presence of increasing amounts of inhibitor (at least 8 points) and 100 muM adenine (P1 mediated) or 100 muM inosine (P2 mediated).	transcription
59312	2	335483	7	NULL	NULL	0	NULL	P2			mediates					adenosine		uptake of			NULL	T. b. brucei bloodstream	0	NULL	NULL	NULL	gw60_molpharmacol_56_6_1162_s_102	10570043	View this table:   [in this window]   [in a new window]     [[ TABLE 1        Ki ]] values for potential inhibitors of P1- and P2-mediated adenosine uptake in  T. b. brucei bloodstream forms    Initial rates of transport were measured by incubating 107 cells for 10 s with [3]adenosine in the presence of increasing amounts of inhibitor (at least 8 points) and 100 muM adenine (P1 mediated) or 100 muM inosine (P2 mediated).	transcription
79117	1	335484	6	NULL	NULL	0	NULL	adenosine	Chemical		is converted to					inosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jneurosci_18_6_1987_s_168	9482785	Thus, the inhibitory effect on synaptic transmission of ATP and gamma-substituted ATP analogs was inhibited (1) by AOPCP, an inhibitor of ecto-5'-nucleotidase, the enzyme that forms adenosine from extracellular adenine nucleotides, (2) by adenosine deaminase, which converts adenosine into its inactive metabolite inosine, and (3) by DPCPX, an adenosine A1 receptor antagonist, whereas (4) it was potentiated by the adenosine uptake inhibitor dipyridamole.	transcription
79118	2	335484	6	NULL	NULL	0	NULL	adenosine deaminase	GP		catalyzes					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_18_6_1987_s_168	9482785	Thus, the inhibitory effect on synaptic transmission of ATP and gamma-substituted ATP analogs was inhibited (1) by AOPCP, an inhibitor of ecto-5'-nucleotidase, the enzyme that forms adenosine from extracellular adenine nucleotides, (2) by adenosine deaminase, which converts adenosine into its inactive metabolite inosine, and (3) by DPCPX, an adenosine A1 receptor antagonist, whereas (4) it was potentiated by the adenosine uptake inhibitor dipyridamole.	transcription
79119	3	335484	6	NULL	NULL	0	NULL	DPCPX	Chemical		is a type of					adenosine A1 receptor antagonist	Chemical				NULL		0	NULL	NULL	NULL	gw60_jneurosci_18_6_1987_s_168	9482785	Thus, the inhibitory effect on synaptic transmission of ATP and gamma-substituted ATP analogs was inhibited (1) by AOPCP, an inhibitor of ecto-5'-nucleotidase, the enzyme that forms adenosine from extracellular adenine nucleotides, (2) by adenosine deaminase, which converts adenosine into its inactive metabolite inosine, and (3) by DPCPX, an adenosine A1 receptor antagonist, whereas (4) it was potentiated by the adenosine uptake inhibitor dipyridamole.	transcription
79120	4	335484	6	NULL	NULL	0	NULL	adenine nucleotides	Chemical		forms					adenosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jneurosci_18_6_1987_s_168	9482785	Thus, the inhibitory effect on synaptic transmission of ATP and gamma-substituted ATP analogs was inhibited (1) by AOPCP, an inhibitor of ecto-5'-nucleotidase, the enzyme that forms adenosine from extracellular adenine nucleotides, (2) by adenosine deaminase, which converts adenosine into its inactive metabolite inosine, and (3) by DPCPX, an adenosine A1 receptor antagonist, whereas (4) it was potentiated by the adenosine uptake inhibitor dipyridamole.	transcription
79121	5	335484	6	NULL	NULL	0	NULL	AOPCP	Chemical		inhibits					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_18_6_1987_s_168	9482785	Thus, the inhibitory effect on synaptic transmission of ATP and gamma-substituted ATP analogs was inhibited (1) by AOPCP, an inhibitor of ecto-5'-nucleotidase, the enzyme that forms adenosine from extracellular adenine nucleotides, (2) by adenosine deaminase, which converts adenosine into its inactive metabolite inosine, and (3) by DPCPX, an adenosine A1 receptor antagonist, whereas (4) it was potentiated by the adenosine uptake inhibitor dipyridamole.	transcription
59313	1	335484	7	NULL	NULL	0	NULL	AOPCP			inhibits					ATP		synaptic transmission of 			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_18_6_1987_s_168	9482785	Thus, the inhibitory effect on synaptic transmission of ATP and gamma-substituted ATP analogs was inhibited (1) by AOPCP, an inhibitor of ecto-5'-nucleotidase, the enzyme that forms adenosine from extracellular adenine nucleotides, (2) by adenosine deaminase, which converts adenosine into its inactive metabolite inosine, and (3) by DPCPX, an adenosine A1 receptor antagonist, whereas (4) it was potentiated by the adenosine uptake inhibitor dipyridamole.	transcription
59314	2	335484	7	NULL	NULL	0	NULL	AOPCP			inhibits					gamma-substituted ATP analogs		synaptic transmission of 			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_18_6_1987_s_168	9482785	Thus, the inhibitory effect on synaptic transmission of ATP and gamma-substituted ATP analogs was inhibited (1) by AOPCP, an inhibitor of ecto-5'-nucleotidase, the enzyme that forms adenosine from extracellular adenine nucleotides, (2) by adenosine deaminase, which converts adenosine into its inactive metabolite inosine, and (3) by DPCPX, an adenosine A1 receptor antagonist, whereas (4) it was potentiated by the adenosine uptake inhibitor dipyridamole.	transcription
59315	3	335484	7	NULL	NULL	0	NULL	AOPCP			an inhibitor of					ecto-5'-nucleotidase					NULL		0	NULL	NULL	NULL	gw60_jneurosci_18_6_1987_s_168	9482785	Thus, the inhibitory effect on synaptic transmission of ATP and gamma-substituted ATP analogs was inhibited (1) by AOPCP, an inhibitor of ecto-5'-nucleotidase, the enzyme that forms adenosine from extracellular adenine nucleotides, (2) by adenosine deaminase, which converts adenosine into its inactive metabolite inosine, and (3) by DPCPX, an adenosine A1 receptor antagonist, whereas (4) it was potentiated by the adenosine uptake inhibitor dipyridamole.	transcription
59316	4	335484	7	NULL	NULL	0	NULL	adenosine			formed from					adenine nucleotides		extracellular			NULL		0	NULL	NULL	NULL	gw60_jneurosci_18_6_1987_s_168	9482785	Thus, the inhibitory effect on synaptic transmission of ATP and gamma-substituted ATP analogs was inhibited (1) by AOPCP, an inhibitor of ecto-5'-nucleotidase, the enzyme that forms adenosine from extracellular adenine nucleotides, (2) by adenosine deaminase, which converts adenosine into its inactive metabolite inosine, and (3) by DPCPX, an adenosine A1 receptor antagonist, whereas (4) it was potentiated by the adenosine uptake inhibitor dipyridamole.	transcription
59317	5	335484	7	NULL	NULL	0	NULL	ecto-5'-nucleotidase			catalyze					statement 4					NULL		0	NULL	NULL	NULL	gw60_jneurosci_18_6_1987_s_168	9482785	Thus, the inhibitory effect on synaptic transmission of ATP and gamma-substituted ATP analogs was inhibited (1) by AOPCP, an inhibitor of ecto-5'-nucleotidase, the enzyme that forms adenosine from extracellular adenine nucleotides, (2) by adenosine deaminase, which converts adenosine into its inactive metabolite inosine, and (3) by DPCPX, an adenosine A1 receptor antagonist, whereas (4) it was potentiated by the adenosine uptake inhibitor dipyridamole.	transcription
59318	6	335484	7	NULL	NULL	0	NULL	adenosine deaminase			inhibits					ATP 		synaptic transmission of 			NULL		0	NULL	NULL	NULL	gw60_jneurosci_18_6_1987_s_168	9482785	Thus, the inhibitory effect on synaptic transmission of ATP and gamma-substituted ATP analogs was inhibited (1) by AOPCP, an inhibitor of ecto-5'-nucleotidase, the enzyme that forms adenosine from extracellular adenine nucleotides, (2) by adenosine deaminase, which converts adenosine into its inactive metabolite inosine, and (3) by DPCPX, an adenosine A1 receptor antagonist, whereas (4) it was potentiated by the adenosine uptake inhibitor dipyridamole.	transcription
59319	7	335484	7	NULL	NULL	0	NULL	adenosine deaminase			inhibits					gamma-substituted ATP analogs		synaptic transmission of 			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_18_6_1987_s_168	9482785	Thus, the inhibitory effect on synaptic transmission of ATP and gamma-substituted ATP analogs was inhibited (1) by AOPCP, an inhibitor of ecto-5'-nucleotidase, the enzyme that forms adenosine from extracellular adenine nucleotides, (2) by adenosine deaminase, which converts adenosine into its inactive metabolite inosine, and (3) by DPCPX, an adenosine A1 receptor antagonist, whereas (4) it was potentiated by the adenosine uptake inhibitor dipyridamole.	transcription
59320	8	335484	7	NULL	NULL	0	NULL	adenosine			converted to					inosine					NULL		0	NULL	NULL	NULL	gw60_jneurosci_18_6_1987_s_168	9482785	Thus, the inhibitory effect on synaptic transmission of ATP and gamma-substituted ATP analogs was inhibited (1) by AOPCP, an inhibitor of ecto-5'-nucleotidase, the enzyme that forms adenosine from extracellular adenine nucleotides, (2) by adenosine deaminase, which converts adenosine into its inactive metabolite inosine, and (3) by DPCPX, an adenosine A1 receptor antagonist, whereas (4) it was potentiated by the adenosine uptake inhibitor dipyridamole.	transcription
59321	9	335484	7	NULL	NULL	0	NULL	adenosine deaminase			catalyze					statement 8					NULL		0	NULL	NULL	NULL	gw60_jneurosci_18_6_1987_s_168	9482785	Thus, the inhibitory effect on synaptic transmission of ATP and gamma-substituted ATP analogs was inhibited (1) by AOPCP, an inhibitor of ecto-5'-nucleotidase, the enzyme that forms adenosine from extracellular adenine nucleotides, (2) by adenosine deaminase, which converts adenosine into its inactive metabolite inosine, and (3) by DPCPX, an adenosine A1 receptor antagonist, whereas (4) it was potentiated by the adenosine uptake inhibitor dipyridamole.	transcription
59322	10	335484	7	NULL	NULL	0	NULL	inosine			is a type of					inactive metabolite					NULL		0	NULL	NULL	NULL	gw60_jneurosci_18_6_1987_s_168	9482785	Thus, the inhibitory effect on synaptic transmission of ATP and gamma-substituted ATP analogs was inhibited (1) by AOPCP, an inhibitor of ecto-5'-nucleotidase, the enzyme that forms adenosine from extracellular adenine nucleotides, (2) by adenosine deaminase, which converts adenosine into its inactive metabolite inosine, and (3) by DPCPX, an adenosine A1 receptor antagonist, whereas (4) it was potentiated by the adenosine uptake inhibitor dipyridamole.	transcription
59323	11	335484	7	NULL	NULL	0	NULL	DPCPX			inhibits					ATP		synaptic transmission of 			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_18_6_1987_s_168	9482785	Thus, the inhibitory effect on synaptic transmission of ATP and gamma-substituted ATP analogs was inhibited (1) by AOPCP, an inhibitor of ecto-5'-nucleotidase, the enzyme that forms adenosine from extracellular adenine nucleotides, (2) by adenosine deaminase, which converts adenosine into its inactive metabolite inosine, and (3) by DPCPX, an adenosine A1 receptor antagonist, whereas (4) it was potentiated by the adenosine uptake inhibitor dipyridamole.	transcription
59324	12	335484	7	NULL	NULL	0	NULL	DPCPX			inhibits					 gamma-substituted ATP analogs		synaptic transmission of 			NULL		0	NULL	NULL	NULL	gw60_jneurosci_18_6_1987_s_168	9482785	Thus, the inhibitory effect on synaptic transmission of ATP and gamma-substituted ATP analogs was inhibited (1) by AOPCP, an inhibitor of ecto-5'-nucleotidase, the enzyme that forms adenosine from extracellular adenine nucleotides, (2) by adenosine deaminase, which converts adenosine into its inactive metabolite inosine, and (3) by DPCPX, an adenosine A1 receptor antagonist, whereas (4) it was potentiated by the adenosine uptake inhibitor dipyridamole.	transcription
59325	13	335484	7	NULL	NULL	0	NULL	DPCPX			is a antagonist of					adenosine A1 receptor 					NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_18_6_1987_s_168	9482785	Thus, the inhibitory effect on synaptic transmission of ATP and gamma-substituted ATP analogs was inhibited (1) by AOPCP, an inhibitor of ecto-5'-nucleotidase, the enzyme that forms adenosine from extracellular adenine nucleotides, (2) by adenosine deaminase, which converts adenosine into its inactive metabolite inosine, and (3) by DPCPX, an adenosine A1 receptor antagonist, whereas (4) it was potentiated by the adenosine uptake inhibitor dipyridamole.	transcription
59326	14	335484	7	NULL	NULL	0	NULL	dipyridamole			potentiate					ATP 		synaptic transmission of 			NULL		0	NULL	NULL	NULL	gw60_jneurosci_18_6_1987_s_168	9482785	Thus, the inhibitory effect on synaptic transmission of ATP and gamma-substituted ATP analogs was inhibited (1) by AOPCP, an inhibitor of ecto-5'-nucleotidase, the enzyme that forms adenosine from extracellular adenine nucleotides, (2) by adenosine deaminase, which converts adenosine into its inactive metabolite inosine, and (3) by DPCPX, an adenosine A1 receptor antagonist, whereas (4) it was potentiated by the adenosine uptake inhibitor dipyridamole.	transcription
59327	15	335484	7	NULL	NULL	0	NULL	dipyridamole			potentiate					gamma-substituted ATP analogs		synaptic transmission of 			NULL		0	NULL	NULL	NULL	gw60_jneurosci_18_6_1987_s_168	9482785	Thus, the inhibitory effect on synaptic transmission of ATP and gamma-substituted ATP analogs was inhibited (1) by AOPCP, an inhibitor of ecto-5'-nucleotidase, the enzyme that forms adenosine from extracellular adenine nucleotides, (2) by adenosine deaminase, which converts adenosine into its inactive metabolite inosine, and (3) by DPCPX, an adenosine A1 receptor antagonist, whereas (4) it was potentiated by the adenosine uptake inhibitor dipyridamole.	transcription
59328	16	335484	7	NULL	NULL	0	NULL	dipyridamole			is an inhibitor of					adenosine uptake					NULL		0	NULL	NULL	NULL	gw60_jneurosci_18_6_1987_s_168	9482785	Thus, the inhibitory effect on synaptic transmission of ATP and gamma-substituted ATP analogs was inhibited (1) by AOPCP, an inhibitor of ecto-5'-nucleotidase, the enzyme that forms adenosine from extracellular adenine nucleotides, (2) by adenosine deaminase, which converts adenosine into its inactive metabolite inosine, and (3) by DPCPX, an adenosine A1 receptor antagonist, whereas (4) it was potentiated by the adenosine uptake inhibitor dipyridamole.	transcription
79122	1	335485	6	NULL	NULL	0	NULL	Fe3+	Chemical		bind					adenine N7	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_43_42495_s_181	12913009	5, whereas binding of Fe3+ to the adenine N7 is favored at neutral pH ( ).	transcription
59329	1	335485	7	NULL	NULL	0	NULL	Fe3+			bind					adenine N7					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_43_42495_s_181	12913009	5, whereas binding of Fe3+ to the adenine N7 is favored at neutral pH ( ).	transcription
59330	2	335485	7	NULL	NULL	0	NULL	neurtral pH			favours					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_43_42495_s_181	12913009	5, whereas binding of Fe3+ to the adenine N7 is favored at neutral pH ( ).	transcription
59331	1	335488	7	NULL	NULL	0	NULL	M.EcoRI			modifies					recognition hexanucleotide				adenine on the 5''-half of	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_35_37049_s_539	15210696	Further, all but M.EcoRI methylate an adenine either at the 3''-end of the site, or the penultimate base, whereas M.EcoRI modifies the adenine on the 5''-half of the recognition hexanucleotide.	transcription
79123	1	335489	6	NULL	NULL	NULL	NULL	GCAP-2/Ca	GP		regulates					RetGC-1	GP		ICD		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_20_11646_s_176	8662612	Regulation of ICD RetGC-1 by GCAP-2/Ca   and Adenine NucleotidesThe catalytic activity of ICD  RetGC-1 is regulated by GCAP-2, Ca , and adenine  nucleotides ( Fig. 5,  B  and  C).	transcription
79124	2	335489	6	NULL	NULL	0	NULL	GCAP-2	GP		regulates					RetGC-1	GP	catalytic activity of	ICD		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_20_11646_s_176	8662612	Regulation of ICD RetGC-1 by GCAP-2/Ca   and Adenine NucleotidesThe catalytic activity of ICD  RetGC-1 is regulated by GCAP-2, Ca , and adenine  nucleotides ( Fig. 5,  B  and  C).	transcription
59332	1	335489	7	NULL	NULL	0	NULL	GCAP-2			regulates					ICD RetGC-1		catalytic activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_20_11646_s_176	8662612	Regulation of ICD RetGC-1 by GCAP-2/Ca   and Adenine NucleotidesThe catalytic activity of ICD  RetGC-1 is regulated by GCAP-2, Ca , and adenine  nucleotides ( Fig. 5,  B  and  C).	transcription
59333	2	335489	7	NULL	NULL	0	NULL	Ca			regulates					ICD RetGC-1		catalytic activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_20_11646_s_176	8662612	Regulation of ICD RetGC-1 by GCAP-2/Ca   and Adenine NucleotidesThe catalytic activity of ICD  RetGC-1 is regulated by GCAP-2, Ca , and adenine  nucleotides ( Fig. 5,  B  and  C).	transcription
59334	3	335489	7	NULL	NULL	0	NULL	adenine nucleotides			regulates					ICD RetGC-1		catalytic activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_20_11646_s_176	8662612	Regulation of ICD RetGC-1 by GCAP-2/Ca   and Adenine NucleotidesThe catalytic activity of ICD  RetGC-1 is regulated by GCAP-2, Ca , and adenine  nucleotides ( Fig. 5,  B  and  C).	transcription
59335	1	335490	7	NULL	NULL	0	NULL	DEPC			mediates					ANF 5''-FS		modification of		adenines at positions -113, -112, -111, -110, and -105 on the + strand	NULL		0	NULL	NULL	NULL	gw60_circulationres_77_6_1060_s_117	7586217	DEPC-mediated modification of adenines at positions -113, -112, -111, -110, and -105 on the + strand of the ANF 5''-FS interfered with complex formation (Fig 5A  , DEPC +), as did modification of adenines -114 and -116 on the - strand (Fig 5A  , DEPC -).	transcription
59336	2	335490	7	NULL	NULL	0	NULL	DEPC			mediates					ANF 5''-FS		modification of		adenines -114 and -116 on the - strand	NULL		0	NULL	NULL	NULL	gw60_circulationres_77_6_1060_s_117	7586217	DEPC-mediated modification of adenines at positions -113, -112, -111, -110, and -105 on the + strand of the ANF 5''-FS interfered with complex formation (Fig 5A  , DEPC +), as did modification of adenines -114 and -116 on the - strand (Fig 5A  , DEPC -).	transcription
79125	1	335491	6	NULL	NULL	0	NULL	AMP	Chemical		bind					Mg2+	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_35_37163_s_186	15210687	In the case of product complex with AMP and Mg2+ ( Fig. 5 A), the adenine was recognized by Ile-19 and Tyr-28* through stacking interactions and adenine N1 made a hydrogen bond with Glu-29*, and adenine N6 made hydrogen bonds with Glu-29* and Gly-104*, although positions of adenine and alpha-phosphate of AMP were located away from residues in the Nudix motif.	transcription
59337	1	335491	7	NULL	NULL	0	NULL	AMP			complex with					Mg2+					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_35_37163_s_186	15210687	In the case of product complex with AMP and Mg2+ ( Fig. 5 A), the adenine was recognized by Ile-19 and Tyr-28* through stacking interactions and adenine N1 made a hydrogen bond with Glu-29*, and adenine N6 made hydrogen bonds with Glu-29* and Gly-104*, although positions of adenine and alpha-phosphate of AMP were located away from residues in the Nudix motif.	transcription
59338	2	335491	7	NULL	NULL	0	NULL	adenine			recognized by					Ile-19					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_35_37163_s_186	15210687	In the case of product complex with AMP and Mg2+ ( Fig. 5 A), the adenine was recognized by Ile-19 and Tyr-28* through stacking interactions and adenine N1 made a hydrogen bond with Glu-29*, and adenine N6 made hydrogen bonds with Glu-29* and Gly-104*, although positions of adenine and alpha-phosphate of AMP were located away from residues in the Nudix motif.	transcription
59339	3	335491	7	NULL	NULL	0	NULL	adenine			recognized by					Tyr-28					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_35_37163_s_186	15210687	In the case of product complex with AMP and Mg2+ ( Fig. 5 A), the adenine was recognized by Ile-19 and Tyr-28* through stacking interactions and adenine N1 made a hydrogen bond with Glu-29*, and adenine N6 made hydrogen bonds with Glu-29* and Gly-104*, although positions of adenine and alpha-phosphate of AMP were located away from residues in the Nudix motif.	transcription
59340	4	335491	7	NULL	NULL	0	NULL	statement 2			through					stacking interactions					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_35_37163_s_186	15210687	In the case of product complex with AMP and Mg2+ ( Fig. 5 A), the adenine was recognized by Ile-19 and Tyr-28* through stacking interactions and adenine N1 made a hydrogen bond with Glu-29*, and adenine N6 made hydrogen bonds with Glu-29* and Gly-104*, although positions of adenine and alpha-phosphate of AMP were located away from residues in the Nudix motif.	transcription
59341	5	335491	7	NULL	NULL	0	NULL	statement 3			through					stacking interactions					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_35_37163_s_186	15210687	In the case of product complex with AMP and Mg2+ ( Fig. 5 A), the adenine was recognized by Ile-19 and Tyr-28* through stacking interactions and adenine N1 made a hydrogen bond with Glu-29*, and adenine N6 made hydrogen bonds with Glu-29* and Gly-104*, although positions of adenine and alpha-phosphate of AMP were located away from residues in the Nudix motif.	transcription
59342	6	335491	7	NULL	NULL	0	NULL	adenine N1			hydrogen bond with					Glu-29					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_35_37163_s_186	15210687	In the case of product complex with AMP and Mg2+ ( Fig. 5 A), the adenine was recognized by Ile-19 and Tyr-28* through stacking interactions and adenine N1 made a hydrogen bond with Glu-29*, and adenine N6 made hydrogen bonds with Glu-29* and Gly-104*, although positions of adenine and alpha-phosphate of AMP were located away from residues in the Nudix motif.	transcription
59343	7	335491	7	NULL	NULL	0	NULL	adenine N6			hydrogen bond with					Gly-104					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_35_37163_s_186	15210687	In the case of product complex with AMP and Mg2+ ( Fig. 5 A), the adenine was recognized by Ile-19 and Tyr-28* through stacking interactions and adenine N1 made a hydrogen bond with Glu-29*, and adenine N6 made hydrogen bonds with Glu-29* and Gly-104*, although positions of adenine and alpha-phosphate of AMP were located away from residues in the Nudix motif.	transcription
59344	1	335492	7	NULL	NULL	0	NULL	adenine 			mutated to				at position 5(-5)	cytosine				at position 5(-5)	NULL		0	NULL	NULL	NULL	gw60_cell_84_5_791_s_174	8625416	By contrast, mutation of  the adenine at position 5(-5) dramatically affects EBNA1 binding; the EBNA1 affinity for its  binding site drops 30-fold if position 5 is changed from an adenine  to a cytosine or a guanine (Ambinder et al., 1990   ).	transcription
59345	2	335492	7	NULL	NULL	0	NULL	adenine			mutated to				at position 5(-5)	guanine				at position 5(-5)	NULL		0	NULL	NULL	NULL	gw60_cell_84_5_791_s_174	8625416	By contrast, mutation of  the adenine at position 5(-5) dramatically affects EBNA1 binding; the EBNA1 affinity for its  binding site drops 30-fold if position 5 is changed from an adenine  to a cytosine or a guanine (Ambinder et al., 1990   ).	transcription
59346	3	335492	7	NULL	NULL	0	NULL	statement 1			affects					EBNA1		binding of			NULL		0	NULL	NULL	NULL	gw60_cell_84_5_791_s_174	8625416	By contrast, mutation of  the adenine at position 5(-5) dramatically affects EBNA1 binding; the EBNA1 affinity for its  binding site drops 30-fold if position 5 is changed from an adenine  to a cytosine or a guanine (Ambinder et al., 1990   ).	transcription
59347	4	335492	7	NULL	NULL	0	NULL	statement 2			affects					EBNA1		binding of			NULL		0	NULL	NULL	NULL	gw60_cell_84_5_791_s_174	8625416	By contrast, mutation of  the adenine at position 5(-5) dramatically affects EBNA1 binding; the EBNA1 affinity for its  binding site drops 30-fold if position 5 is changed from an adenine  to a cytosine or a guanine (Ambinder et al., 1990   ).	transcription
59348	1	335493	7	NULL	NULL	0	NULL	common polymorphism			affect					MMP-3		promoter			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_11_1254_s_29	12750310	A naturally occurring and common polymorphism affects the MMP-3 promoter, where either 5 or 6 consecutive adenines (5A/6A) alter transcription factor binding and affect MMP-3 promoter activity.	transcription
59349	2	335493	7	NULL	NULL	0	NULL	5A			alter					transcription factor		binding of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_11_1254_s_29	12750310	A naturally occurring and common polymorphism affects the MMP-3 promoter, where either 5 or 6 consecutive adenines (5A/6A) alter transcription factor binding and affect MMP-3 promoter activity.	transcription
59350	3	335493	7	NULL	NULL	0	NULL	6A			alter					transcription factor		binding of			NULL		0	NULL	NULL	NULL	gw70_circulationres_92_11_1254_s_29	12750310	A naturally occurring and common polymorphism affects the MMP-3 promoter, where either 5 or 6 consecutive adenines (5A/6A) alter transcription factor binding and affect MMP-3 promoter activity.	transcription
59351	4	335493	7	NULL	NULL	0	NULL	5A			affect					MMP-3		activity of		promoter	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_11_1254_s_29	12750310	A naturally occurring and common polymorphism affects the MMP-3 promoter, where either 5 or 6 consecutive adenines (5A/6A) alter transcription factor binding and affect MMP-3 promoter activity.	transcription
59352	5	335493	7	NULL	NULL	0	NULL	6A			affect					MMP-3		activity of		promoter	NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_11_1254_s_29	12750310	A naturally occurring and common polymorphism affects the MMP-3 promoter, where either 5 or 6 consecutive adenines (5A/6A) alter transcription factor binding and affect MMP-3 promoter activity.	transcription
59353	6	335493	7	NULL	NULL	0	NULL	5A			is					5 consecutive adenines					NULL		NULL	NULL	NULL	NULL	gw70_circulationres_92_11_1254_s_29	12750310	A naturally occurring and common polymorphism affects the MMP-3 promoter, where either 5 or 6 consecutive adenines (5A/6A) alter transcription factor binding and affect MMP-3 promoter activity.	transcription
59361	7	335493	7	NULL	NULL	0	NULL	6A			is					6 consecutive adenines					NULL		0	NULL	NULL	NULL	gw70_circulationres_92_11_1254_s_29	12750310	A naturally occurring and common polymorphism affects the MMP-3 promoter, where either 5 or 6 consecutive adenines (5A/6A) alter transcription factor binding and affect MMP-3 promoter activity.	transcription
79126	1	335495	6	NULL	NULL	0	NULL	PABPN1	GP		recognizes					adenine bases	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_19_16916_s_413	12637556	The selection experiment (Fig.  5) suggests that PABPN1 recognizes adenine bases in a specific fashion throughout its  binding site.	transcription
59366	1	335495	7	NULL	NULL	0	NULL	PABPN1			recognizes		specifically			adenine bases				binding site	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_19_16916_s_413	12637556	The selection experiment (Fig.  5) suggests that PABPN1 recognizes adenine bases in a specific fashion throughout its  binding site.	transcription
79127	1	335496	6	NULL	NULL	0	NULL	BVR	GP		phosphorylates					IRS	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_102_20_7109_s_230	15870194	A point mutation introduced in the adenine-binding domain ( ) of BVR (GXGXXG) significantly decreased phosphorylation of IRS by BVR ( Fig. 5).	transcription
79128	2	335496	6	NULL	NULL	0	NULL	BVR	GP	mutation of 	decreases during					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_102_20_7109_s_230	15870194	A point mutation introduced in the adenine-binding domain ( ) of BVR (GXGXXG) significantly decreased phosphorylation of IRS by BVR ( Fig. 5).	transcription
59367	1	335496	7	NULL	NULL	0	NULL	BVR			phosphorylates					IRS					NULL		0	NULL	NULL	NULL	gw70_pnas_102_20_7109_s_230	15870194	A point mutation introduced in the adenine-binding domain ( ) of BVR (GXGXXG) significantly decreased phosphorylation of IRS by BVR ( Fig. 5).	transcription
59368	2	335496	7	NULL	NULL	0	NULL	BVR		point mutant	decrease		significantly	adenine-binding domain GXGXXG		statement 1					NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_20_7109_s_230	15870194	A point mutation introduced in the adenine-binding domain ( ) of BVR (GXGXXG) significantly decreased phosphorylation of IRS by BVR ( Fig. 5).	transcription
59369	1	335497	7	NULL	NULL	0	NULL	Stx1			complex with					ribosome					NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_12_2383_s_95	10871371	From such increase a value of  Kiu of 66 muM for the binding of adenine to the Stx1 - ribosome complex was obtained in the previous paper ( 5).	transcription
59370	2	335497	7	NULL	NULL	0	NULL	adenine			bind					statement 1					NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_12_2383_s_95	10871371	From such increase a value of  Kiu of 66 muM for the binding of adenine to the Stx1 - ribosome complex was obtained in the previous paper ( 5).	transcription
79129	1	335498	6	NULL	NULL	0	NULL	BAS2p	GP		plays a role in					adenine	Chemical	regulation of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_47_29637_s_34	8939895	Finally, together with BAS1p, BAS2p is involved in the adenine regulation of either purine ( 5) or amino acid biosynthetic genes.	transcription
79130	2	335498	6	NULL	NULL	0	NULL	statement 1	Process		occurs together with					BAS1p	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_47_29637_s_34	8939895	Finally, together with BAS1p, BAS2p is involved in the adenine regulation of either purine ( 5) or amino acid biosynthetic genes.	transcription
59371	1	335498	7	NULL	NULL	0	NULL	BAS1p			is involved in					adenine		regulation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_47_29637_s_34	8939895	Finally, together with BAS1p, BAS2p is involved in the adenine regulation of either purine ( 5) or amino acid biosynthetic genes.	transcription
59372	2	335498	7	NULL	NULL	0	NULL	BAS2p			is involved in					adenine		regulation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_47_29637_s_34	8939895	Finally, together with BAS1p, BAS2p is involved in the adenine regulation of either purine ( 5) or amino acid biosynthetic genes.	transcription
59373	3	335498	7	NULL	NULL	0	NULL	statement 1			occur simulataneous with					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_47_29637_s_34	8939895	Finally, together with BAS1p, BAS2p is involved in the adenine regulation of either purine ( 5) or amino acid biosynthetic genes.	transcription
59374	4	335498	7	NULL	NULL	0	NULL	BAS1p			is involved in					amino acid biosynthetic genes		regulation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_47_29637_s_34	8939895	Finally, together with BAS1p, BAS2p is involved in the adenine regulation of either purine ( 5) or amino acid biosynthetic genes.	transcription
59375	5	335498	7	NULL	NULL	0	NULL	BAS2p			is involved in					amino acid biosynthetic genes		regulation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_47_29637_s_34	8939895	Finally, together with BAS1p, BAS2p is involved in the adenine regulation of either purine ( 5) or amino acid biosynthetic genes.	transcription
59376	6	335498	7	NULL	NULL	0	NULL	statement 4			occur simulataneous with					statement 5					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_47_29637_s_34	8939895	Finally, together with BAS1p, BAS2p is involved in the adenine regulation of either purine ( 5) or amino acid biosynthetic genes.	transcription
59377	7	335498	7	NULL	NULL	0	NULL	statement 3			is an alternative to					statement 6					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_47_29637_s_34	8939895	Finally, together with BAS1p, BAS2p is involved in the adenine regulation of either purine ( 5) or amino acid biosynthetic genes.	transcription
79131	1	335499	6	NULL	NULL	0	NULL	adenine nucleotides	Chemical		regulates					5 ''-nucleotidase	GP				NULL	rat heart	0	NULL	NULL	NULL	gw60_jpharmacolexpther_298_1_71_s_268	11408527	Sullivan JM and Alpers JB (1971) In vitro regulation of rat heart 5 ''-nucleotidaseby adenine nucleotides and magnesium.	transcription
59378	1	335499	7	NULL	NULL	0	NULL	adenine nucleotides			regulates					5 ''-nucleotidase		rat;;heart			NULL	in vitro	0	NULL	NULL	NULL	gw60_jpharmacolexpther_298_1_71_s_268	11408527	Sullivan JM and Alpers JB (1971) In vitro regulation of rat heart 5 ''-nucleotidaseby adenine nucleotides and magnesium.	transcription
59379	2	335499	7	NULL	NULL	0	NULL	magnesium			regulates					5 ''-nucleotidase		rat;;heart			NULL	in vitro	0	NULL	NULL	NULL	gw60_jpharmacolexpther_298_1_71_s_268	11408527	Sullivan JM and Alpers JB (1971) In vitro regulation of rat heart 5 ''-nucleotidaseby adenine nucleotides and magnesium.	transcription
79132	1	335501	6	NULL	NULL	0	NULL	Stx-1	Chemical		induces					adenine	Chemical	release of			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_12_2383_s_80	10871371	Similarly, 4-APP was more effective than adenine in protecting the DNA substrate from the [3]adenine release induced by 200 nM Stx1 (38  plus-or-minus  9 pmol,  n = 5).	transcription
79133	2	335501	6	NULL	NULL	0	NULL	APP	Chemical		protects from					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_12_2383_s_80	10871371	Similarly, 4-APP was more effective than adenine in protecting the DNA substrate from the [3]adenine release induced by 200 nM Stx1 (38  plus-or-minus  9 pmol,  n = 5).	transcription
59380	2	335501	7	NULL	NULL	0	NULL	Stx1 			induce					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_12_2383_s_80	10871371	Similarly, 4-APP was more effective than adenine in protecting the DNA substrate from the [3]adenine release induced by 200 nM Stx1 (38  plus-or-minus  9 pmol,  n = 5).	transcription
59381	3	335501	7	NULL	NULL	0	NULL	4-APP			protects					statement 2					NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_12_2383_s_80	10871371	Similarly, 4-APP was more effective than adenine in protecting the DNA substrate from the [3]adenine release induced by 200 nM Stx1 (38  plus-or-minus  9 pmol,  n = 5).	transcription
59382	1	335501	7	NULL	NULL	0	NULL	adenine			released from					DNA substrate					NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_12_2383_s_80	10871371	Similarly, 4-APP was more effective than adenine in protecting the DNA substrate from the [3]adenine release induced by 200 nM Stx1 (38  plus-or-minus  9 pmol,  n = 5).	transcription
59383	4	335501	7	NULL	NULL	0	NULL	adenine			protects					statement 2					NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_12_2383_s_80	10871371	Similarly, 4-APP was more effective than adenine in protecting the DNA substrate from the [3]adenine release induced by 200 nM Stx1 (38  plus-or-minus  9 pmol,  n = 5).	transcription
59384	5	335501	7	NULL	NULL	0	NULL	statement 3			more effective than					statement 4					NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_12_2383_s_80	10871371	Similarly, 4-APP was more effective than adenine in protecting the DNA substrate from the [3]adenine release induced by 200 nM Stx1 (38  plus-or-minus  9 pmol,  n = 5).	transcription
79134	1	335503	6	NULL	NULL	0	NULL	NADH	Chemical		bind					Th	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10103_s_7	8626568	NADH and reduced acetylpyridine adenine  dinucleotide bound tightly to Th , whereas  NAD , oxidized acetylpyridine adenine dinucleotide,  deamino-NADH, 5``-AMP and adenosine bound less tightly.	transcription
79135	2	335503	6	NULL	NULL	0	NULL	acetylpyridine adenine dinucleotide	Chemical	reduced	bind					Th	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10103_s_7	8626568	NADH and reduced acetylpyridine adenine  dinucleotide bound tightly to Th , whereas  NAD , oxidized acetylpyridine adenine dinucleotide,  deamino-NADH, 5``-AMP and adenosine bound less tightly.	transcription
79136	3	335503	6	NULL	NULL	0	NULL	NAD	Chemical		bind					Th	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10103_s_7	8626568	NADH and reduced acetylpyridine adenine  dinucleotide bound tightly to Th , whereas  NAD , oxidized acetylpyridine adenine dinucleotide,  deamino-NADH, 5``-AMP and adenosine bound less tightly.	transcription
79137	4	335503	6	NULL	NULL	0	NULL	acetylpyridine adenine dinucleotide	Chemical	oxidized	bind					Th	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10103_s_7	8626568	NADH and reduced acetylpyridine adenine  dinucleotide bound tightly to Th , whereas  NAD , oxidized acetylpyridine adenine dinucleotide,  deamino-NADH, 5``-AMP and adenosine bound less tightly.	transcription
79138	5	335503	6	NULL	NULL	0	NULL	deamino-NADH	Chemical		bind					Th	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10103_s_7	8626568	NADH and reduced acetylpyridine adenine  dinucleotide bound tightly to Th , whereas  NAD , oxidized acetylpyridine adenine dinucleotide,  deamino-NADH, 5``-AMP and adenosine bound less tightly.	transcription
79139	6	335503	6	NULL	NULL	0	NULL	AMP	Chemical		bind					Th	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10103_s_7	8626568	NADH and reduced acetylpyridine adenine  dinucleotide bound tightly to Th , whereas  NAD , oxidized acetylpyridine adenine dinucleotide,  deamino-NADH, 5``-AMP and adenosine bound less tightly.	transcription
79140	7	335503	6	NULL	NULL	0	NULL	adenosine	Chemical		bind					Th	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10103_s_7	8626568	NADH and reduced acetylpyridine adenine  dinucleotide bound tightly to Th , whereas  NAD , oxidized acetylpyridine adenine dinucleotide,  deamino-NADH, 5``-AMP and adenosine bound less tightly.	transcription
59619	1	335503	7	NULL	NULL	0	NULL	NADH	Chemical		bind		tightly			Th	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10103_s_7	8626568	NADH and reduced acetylpyridine adenine  dinucleotide bound tightly to Th , whereas  NAD , oxidized acetylpyridine adenine dinucleotide,  deamino-NADH, 5``-AMP and adenosine bound less tightly.	transcription
59620	2	335503	7	NULL	NULL	0	NULL	acetylpyridine adenine dinucleotide	Chemical	reduced	bind		tightly			Th	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_17_10103_s_7	8626568	NADH and reduced acetylpyridine adenine  dinucleotide bound tightly to Th , whereas  NAD , oxidized acetylpyridine adenine dinucleotide,  deamino-NADH, 5``-AMP and adenosine bound less tightly.	transcription
59621	3	335503	7	NULL	NULL	0	NULL	NAD	Chemical		bind		less tightly			Th	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10103_s_7	8626568	NADH and reduced acetylpyridine adenine  dinucleotide bound tightly to Th , whereas  NAD , oxidized acetylpyridine adenine dinucleotide,  deamino-NADH, 5``-AMP and adenosine bound less tightly.	transcription
59622	4	335503	7	NULL	NULL	0	NULL	acetylpyridine adenine dinucleotide	Chemical	oxidized	bind		less tightly			Th	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10103_s_7	8626568	NADH and reduced acetylpyridine adenine  dinucleotide bound tightly to Th , whereas  NAD , oxidized acetylpyridine adenine dinucleotide,  deamino-NADH, 5``-AMP and adenosine bound less tightly.	transcription
59623	5	335503	7	NULL	NULL	0	NULL	deamino-NADH	Chemical		bind		less tightly			Th	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10103_s_7	8626568	NADH and reduced acetylpyridine adenine  dinucleotide bound tightly to Th , whereas  NAD , oxidized acetylpyridine adenine dinucleotide,  deamino-NADH, 5``-AMP and adenosine bound less tightly.	transcription
59624	6	335503	7	NULL	NULL	0	NULL	 5``-AMP	Chemical		bind		less tightly			Th	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10103_s_7	8626568	NADH and reduced acetylpyridine adenine  dinucleotide bound tightly to Th , whereas  NAD , oxidized acetylpyridine adenine dinucleotide,  deamino-NADH, 5``-AMP and adenosine bound less tightly.	transcription
59625	7	335503	7	NULL	NULL	0	NULL	adenosine 	Chemical		bind		less tightly			Th	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10103_s_7	8626568	NADH and reduced acetylpyridine adenine  dinucleotide bound tightly to Th , whereas  NAD , oxidized acetylpyridine adenine dinucleotide,  deamino-NADH, 5``-AMP and adenosine bound less tightly.	transcription
79141	1	335505	6	NULL	NULL	0	NULL	adenine nucleotides	Chemical		inhibits					NK cell	cell	proliferation of 			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-immunol_162_12_10358189_s_5	10358189	Adenine nucleotides inhibited NK cell proliferation, with ATP = ADP >  5''-adenylylimidodiphosphate > AMP = adenosine; ADP-ribose and nicotinamide  adenine dinucleotide, but not nicotinamide or UTP, caused a dose-dependent  suppression of thymidine uptake.	transcription
59626	1	335505	7	NULL	NULL	0	NULL	Adenine nucleotides	NucleicAcid		inhibit					NK cell	Cell	cell proliferation of			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-immunol_162_12_10358189_s_5	10358189	Adenine nucleotides inhibited NK cell proliferation, with ATP = ADP >  5''-adenylylimidodiphosphate > AMP = adenosine; ADP-ribose and nicotinamide  adenine dinucleotide, but not nicotinamide or UTP, caused a dose-dependent  suppression of thymidine uptake.	transcription
59627	2	335505	7	NULL	NULL	0	NULL	ADP-ribose	NucleicAcid		suppress		dose-dependently			thymidine	NucleicAcid	uptake of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-immunol_162_12_10358189_s_5	10358189	Adenine nucleotides inhibited NK cell proliferation, with ATP = ADP >  5''-adenylylimidodiphosphate > AMP = adenosine; ADP-ribose and nicotinamide  adenine dinucleotide, but not nicotinamide or UTP, caused a dose-dependent  suppression of thymidine uptake.	transcription
59628	3	335505	7	NULL	NULL	0	NULL	nicotinamide adenine dinucleotide	Chemical		suppress		dose-dependently			thymidine	NucleicAcid	uptake of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-immunol_162_12_10358189_s_5	10358189	Adenine nucleotides inhibited NK cell proliferation, with ATP = ADP >  5''-adenylylimidodiphosphate > AMP = adenosine; ADP-ribose and nicotinamide  adenine dinucleotide, but not nicotinamide or UTP, caused a dose-dependent  suppression of thymidine uptake.	transcription
59629	4	335505	7	NULL	NULL	0	NULL	nicotinamide	Chemical		does not suppress					thymidine	NucleicAcid	uptake of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_j-immunol_162_12_10358189_s_5	10358189	Adenine nucleotides inhibited NK cell proliferation, with ATP = ADP >  5''-adenylylimidodiphosphate > AMP = adenosine; ADP-ribose and nicotinamide  adenine dinucleotide, but not nicotinamide or UTP, caused a dose-dependent  suppression of thymidine uptake.	transcription
59630	5	335505	7	NULL	NULL	0	NULL	UTP	NucleicAcid		does not suppress					thymidine	NucleicAcid	uptake of			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_j-immunol_162_12_10358189_s_5	10358189	Adenine nucleotides inhibited NK cell proliferation, with ATP = ADP >  5''-adenylylimidodiphosphate > AMP = adenosine; ADP-ribose and nicotinamide  adenine dinucleotide, but not nicotinamide or UTP, caused a dose-dependent  suppression of thymidine uptake.	transcription
79142	1	335506	6	NULL	NULL	0	NULL	Allopurinol	Chemical		inhibits					adenine	Chemical	transport of			NULL		0	NULL	NULL	NULL	gw70_molpharmacol_63_4_814_s_48	12644582	The adenine transporter generally displayed far higher affinity for nucleobases than for their corresponding nucleosides, as illustrated in Fig.  1B for adenine and adenosine, which displayed a  Ki value of >5 mM. Allopurinol was a moderately effective inhibitor of [3]adenine transport (Fig.  1B) with a  Ki of 56  plus-or-minus  2 muM ( n = 3).	transcription
59631	1	335506	7	NULL	NULL	0	NULL	adenine transporter	GP		affinity for					adenine	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_63_4_814_s_48	12644582	The adenine transporter generally displayed far higher affinity for nucleobases than for their corresponding nucleosides, as illustrated in Fig.  1B for adenine and adenosine, which displayed a  Ki value of >5 mM. Allopurinol was a moderately effective inhibitor of [3]adenine transport (Fig.  1B) with a  Ki of 56  plus-or-minus  2 muM ( n = 3).	transcription
59632	2	335506	7	NULL	NULL	0	NULL	adenine transporter	GP		affinity for					adenosine	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_63_4_814_s_48	12644582	The adenine transporter generally displayed far higher affinity for nucleobases than for their corresponding nucleosides, as illustrated in Fig.  1B for adenine and adenosine, which displayed a  Ki value of >5 mM. Allopurinol was a moderately effective inhibitor of [3]adenine transport (Fig.  1B) with a  Ki of 56  plus-or-minus  2 muM ( n = 3).	transcription
59633	3	335506	7	NULL	NULL	0	NULL	statement 1	Process	affinity of	is higher than					statement 2	Process	affinity of			NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_63_4_814_s_48	12644582	The adenine transporter generally displayed far higher affinity for nucleobases than for their corresponding nucleosides, as illustrated in Fig.  1B for adenine and adenosine, which displayed a  Ki value of >5 mM. Allopurinol was a moderately effective inhibitor of [3]adenine transport (Fig.  1B) with a  Ki of 56  plus-or-minus  2 muM ( n = 3).	transcription
59634	4	335506	7	NULL	NULL	0	NULL	Allopurinol	Chemical		inhibitor of		effective			adenine transport	GP				NULL		0	NULL	NULL	NULL	gw70_molpharmacol_63_4_814_s_48	12644582	The adenine transporter generally displayed far higher affinity for nucleobases than for their corresponding nucleosides, as illustrated in Fig.  1B for adenine and adenosine, which displayed a  Ki value of >5 mM. Allopurinol was a moderately effective inhibitor of [3]adenine transport (Fig.  1B) with a  Ki of 56  plus-or-minus  2 muM ( n = 3).	transcription
59635	7	335507	7	NULL	NULL	0	NULL	adenine	NucleicAcid		protects 					U31	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2104_s_257	11705996	Three unpaired nucleotides (U31, U33, and G35) of the first loop (loop I) are clearly protected by adenine against single strand-specific RNase attack, either because of a structural stabilization induced by adenine or simply because they interact directly with the adenine target (Fig.  5).	transcription
59636	8	335507	7	NULL	NULL	0	NULL	adenine	NucleicAcid		protects					U33	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2104_s_257	11705996	Three unpaired nucleotides (U31, U33, and G35) of the first loop (loop I) are clearly protected by adenine against single strand-specific RNase attack, either because of a structural stabilization induced by adenine or simply because they interact directly with the adenine target (Fig.  5).	transcription
59637	9	335507	7	NULL	NULL	0	NULL	adenine	NucleicAcid		protects					G35	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2104_s_257	11705996	Three unpaired nucleotides (U31, U33, and G35) of the first loop (loop I) are clearly protected by adenine against single strand-specific RNase attack, either because of a structural stabilization induced by adenine or simply because they interact directly with the adenine target (Fig.  5).	transcription
59638	4	335507	7	NULL	NULL	0	NULL	U31	NucleicAcid		belongs to									loop I	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2104_s_257	11705996	Three unpaired nucleotides (U31, U33, and G35) of the first loop (loop I) are clearly protected by adenine against single strand-specific RNase attack, either because of a structural stabilization induced by adenine or simply because they interact directly with the adenine target (Fig.  5).	transcription
59639	5	335507	7	NULL	NULL	0	NULL	U33	NucleicAcid		belongs to									Ioop I	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_3_2104_s_257	11705996	Three unpaired nucleotides (U31, U33, and G35) of the first loop (loop I) are clearly protected by adenine against single strand-specific RNase attack, either because of a structural stabilization induced by adenine or simply because they interact directly with the adenine target (Fig.  5).	transcription
59640	6	335507	7	NULL	NULL	0	NULL	G35	NucleicAcid		belongs to									loop I	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_3_2104_s_257	11705996	Three unpaired nucleotides (U31, U33, and G35) of the first loop (loop I) are clearly protected by adenine against single strand-specific RNase attack, either because of a structural stabilization induced by adenine or simply because they interact directly with the adenine target (Fig.  5).	transcription
59641	1	335507	7	NULL	NULL	0	NULL	single strand-specific RNase 	GP		attack					U31	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2104_s_257	11705996	Three unpaired nucleotides (U31, U33, and G35) of the first loop (loop I) are clearly protected by adenine against single strand-specific RNase attack, either because of a structural stabilization induced by adenine or simply because they interact directly with the adenine target (Fig.  5).	transcription
59642	2	335507	7	NULL	NULL	0	NULL	single strand-specific RNase 	GP		attack					U33	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2104_s_257	11705996	Three unpaired nucleotides (U31, U33, and G35) of the first loop (loop I) are clearly protected by adenine against single strand-specific RNase attack, either because of a structural stabilization induced by adenine or simply because they interact directly with the adenine target (Fig.  5).	transcription
59643	3	335507	7	NULL	NULL	0	NULL	single strand-specific RNase 	GP		attack					G35	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2104_s_257	11705996	Three unpaired nucleotides (U31, U33, and G35) of the first loop (loop I) are clearly protected by adenine against single strand-specific RNase attack, either because of a structural stabilization induced by adenine or simply because they interact directly with the adenine target (Fig.  5).	transcription
59644	10	335507	7	NULL	NULL	0	NULL	statement 7	Process		protected from					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_3_2104_s_257	11705996	Three unpaired nucleotides (U31, U33, and G35) of the first loop (loop I) are clearly protected by adenine against single strand-specific RNase attack, either because of a structural stabilization induced by adenine or simply because they interact directly with the adenine target (Fig.  5).	transcription
59645	11	335507	7	NULL	NULL	0	NULL	statement 8	Process		protected from					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2104_s_257	11705996	Three unpaired nucleotides (U31, U33, and G35) of the first loop (loop I) are clearly protected by adenine against single strand-specific RNase attack, either because of a structural stabilization induced by adenine or simply because they interact directly with the adenine target (Fig.  5).	transcription
59646	12	335507	7	NULL	NULL	0	NULL	statement 9	Process		protected from					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_3_2104_s_257	11705996	Three unpaired nucleotides (U31, U33, and G35) of the first loop (loop I) are clearly protected by adenine against single strand-specific RNase attack, either because of a structural stabilization induced by adenine or simply because they interact directly with the adenine target (Fig.  5).	transcription
59647	13	335507	7	NULL	NULL	0	NULL	adenine	NucleicAcid		induce					U31	NucleicAcid	structural stabilization of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2104_s_257	11705996	Three unpaired nucleotides (U31, U33, and G35) of the first loop (loop I) are clearly protected by adenine against single strand-specific RNase attack, either because of a structural stabilization induced by adenine or simply because they interact directly with the adenine target (Fig.  5).	transcription
59648	14	335507	7	NULL	NULL	0	NULL	statement 10	Process		because of					statement 13	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2104_s_257	11705996	Three unpaired nucleotides (U31, U33, and G35) of the first loop (loop I) are clearly protected by adenine against single strand-specific RNase attack, either because of a structural stabilization induced by adenine or simply because they interact directly with the adenine target (Fig.  5).	transcription
59649	15	335507	7	NULL	NULL	0	NULL	adenine	NucleicAcid		induce					U33	NucleicAcid	structural stabilization of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2104_s_257	11705996	Three unpaired nucleotides (U31, U33, and G35) of the first loop (loop I) are clearly protected by adenine against single strand-specific RNase attack, either because of a structural stabilization induced by adenine or simply because they interact directly with the adenine target (Fig.  5).	transcription
59650	16	335507	7	NULL	NULL	0	NULL	statement 11	Process		because of					statement 15	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2104_s_257	11705996	Three unpaired nucleotides (U31, U33, and G35) of the first loop (loop I) are clearly protected by adenine against single strand-specific RNase attack, either because of a structural stabilization induced by adenine or simply because they interact directly with the adenine target (Fig.  5).	transcription
59651	17	335507	7	NULL	NULL	0	NULL	adenine	NucleicAcid		induce					G35	NucleicAcid	structural stabilization of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_3_2104_s_257	11705996	Three unpaired nucleotides (U31, U33, and G35) of the first loop (loop I) are clearly protected by adenine against single strand-specific RNase attack, either because of a structural stabilization induced by adenine or simply because they interact directly with the adenine target (Fig.  5).	transcription
59652	18	335507	7	NULL	NULL	0	NULL	statement 12	Process		because of					statement 17	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_3_2104_s_257	11705996	Three unpaired nucleotides (U31, U33, and G35) of the first loop (loop I) are clearly protected by adenine against single strand-specific RNase attack, either because of a structural stabilization induced by adenine or simply because they interact directly with the adenine target (Fig.  5).	transcription
59653	19	335507	7	NULL	NULL	0	NULL	U31	NucleicAcid		interact with		directly			adenine target	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_3_2104_s_257	11705996	Three unpaired nucleotides (U31, U33, and G35) of the first loop (loop I) are clearly protected by adenine against single strand-specific RNase attack, either because of a structural stabilization induced by adenine or simply because they interact directly with the adenine target (Fig.  5).	transcription
59654	20	335507	7	NULL	NULL	0	NULL	U33	NucleicAcid		interact with		directly			adenine target	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_3_2104_s_257	11705996	Three unpaired nucleotides (U31, U33, and G35) of the first loop (loop I) are clearly protected by adenine against single strand-specific RNase attack, either because of a structural stabilization induced by adenine or simply because they interact directly with the adenine target (Fig.  5).	transcription
59655	21	335507	7	NULL	NULL	0	NULL	G35	NucleicAcid		interact with		directly			adenine target	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_3_2104_s_257	11705996	Three unpaired nucleotides (U31, U33, and G35) of the first loop (loop I) are clearly protected by adenine against single strand-specific RNase attack, either because of a structural stabilization induced by adenine or simply because they interact directly with the adenine target (Fig.  5).	transcription
59656	22	335507	7	NULL	NULL	0	NULL	statement 10	Process		because of					statement 19	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_3_2104_s_257	11705996	Three unpaired nucleotides (U31, U33, and G35) of the first loop (loop I) are clearly protected by adenine against single strand-specific RNase attack, either because of a structural stabilization induced by adenine or simply because they interact directly with the adenine target (Fig.  5).	transcription
59657	23	335507	7	NULL	NULL	0	NULL	statement 11	Process		because of					statement 20	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_3_2104_s_257	11705996	Three unpaired nucleotides (U31, U33, and G35) of the first loop (loop I) are clearly protected by adenine against single strand-specific RNase attack, either because of a structural stabilization induced by adenine or simply because they interact directly with the adenine target (Fig.  5).	transcription
59658	24	335507	7	NULL	NULL	0	NULL	statement 12	Process		because of					statement 21	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_3_2104_s_257	11705996	Three unpaired nucleotides (U31, U33, and G35) of the first loop (loop I) are clearly protected by adenine against single strand-specific RNase attack, either because of a structural stabilization induced by adenine or simply because they interact directly with the adenine target (Fig.  5).	transcription
59659	25	335507	7	NULL	NULL	0	NULL	statement 14	Process		is an alternative to					statement 22	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_3_2104_s_257	11705996	Three unpaired nucleotides (U31, U33, and G35) of the first loop (loop I) are clearly protected by adenine against single strand-specific RNase attack, either because of a structural stabilization induced by adenine or simply because they interact directly with the adenine target (Fig.  5).	transcription
59660	26	335507	7	NULL	NULL	0	NULL	statement 16	Process		is an alternative to					statement 23	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_3_2104_s_257	11705996	Three unpaired nucleotides (U31, U33, and G35) of the first loop (loop I) are clearly protected by adenine against single strand-specific RNase attack, either because of a structural stabilization induced by adenine or simply because they interact directly with the adenine target (Fig.  5).	transcription
59661	27	335507	7	NULL	NULL	0	NULL	statement 18	Process		is an alternative to					statement 24	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_3_2104_s_257	11705996	Three unpaired nucleotides (U31, U33, and G35) of the first loop (loop I) are clearly protected by adenine against single strand-specific RNase attack, either because of a structural stabilization induced by adenine or simply because they interact directly with the adenine target (Fig.  5).	transcription
59662	28	335507	7	NULL	NULL	0	NULL	U31	NucleicAcid		is a type of					unpaired nucleotide	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_3_2104_s_257	11705996	Three unpaired nucleotides (U31, U33, and G35) of the first loop (loop I) are clearly protected by adenine against single strand-specific RNase attack, either because of a structural stabilization induced by adenine or simply because they interact directly with the adenine target (Fig.  5).	transcription
59663	29	335507	7	NULL	NULL	0	NULL	U33	NucleicAcid		is a type of					unpaired nucleotide	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_3_2104_s_257	11705996	Three unpaired nucleotides (U31, U33, and G35) of the first loop (loop I) are clearly protected by adenine against single strand-specific RNase attack, either because of a structural stabilization induced by adenine or simply because they interact directly with the adenine target (Fig.  5).	transcription
59664	30	335507	7	NULL	NULL	0	NULL	G35	NucleicAcid		is a type of					unpaired nucleotide	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_3_2104_s_257	11705996	Three unpaired nucleotides (U31, U33, and G35) of the first loop (loop I) are clearly protected by adenine against single strand-specific RNase attack, either because of a structural stabilization induced by adenine or simply because they interact directly with the adenine target (Fig.  5).	transcription
79143	1	335508	6	NULL	NULL	0	NULL	SAH	GP		forms					SRH	GP				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_13_3450_s_43	12057938	Pfs catalyzes two reactions in bacterial cells: the formation of  S-ribosylhomocysteine (SRH) from  S-adenosylhomocysteine (SAH) to release adenine and the production of 5''-methylthioribose (MTR) from 5''-methylthioadenosine (MTA), also releasing adenine ( 11,  19,  28).	transcription
79144	2	335508	6	NULL	NULL	0	NULL	SAH	GP		is					S-adenosylhomocysteine	GP				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_13_3450_s_43	12057938	Pfs catalyzes two reactions in bacterial cells: the formation of  S-ribosylhomocysteine (SRH) from  S-adenosylhomocysteine (SAH) to release adenine and the production of 5''-methylthioribose (MTR) from 5''-methylthioadenosine (MTA), also releasing adenine ( 11,  19,  28).	transcription
79145	3	335508	6	NULL	NULL	0	NULL	SRH	GP		is					S-ribosylhomocysteine	GP				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_13_3450_s_43	12057938	Pfs catalyzes two reactions in bacterial cells: the formation of  S-ribosylhomocysteine (SRH) from  S-adenosylhomocysteine (SAH) to release adenine and the production of 5''-methylthioribose (MTR) from 5''-methylthioadenosine (MTA), also releasing adenine ( 11,  19,  28).	transcription
79146	4	335508	6	NULL	NULL	0	NULL	Pf	GP		catalyzes					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_13_3450_s_43	12057938	Pfs catalyzes two reactions in bacterial cells: the formation of  S-ribosylhomocysteine (SRH) from  S-adenosylhomocysteine (SAH) to release adenine and the production of 5''-methylthioribose (MTR) from 5''-methylthioadenosine (MTA), also releasing adenine ( 11,  19,  28).	transcription
79147	5	335508	6	NULL	NULL	0	NULL	statement 1	Process		releases					adenine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_13_3450_s_43	12057938	Pfs catalyzes two reactions in bacterial cells: the formation of  S-ribosylhomocysteine (SRH) from  S-adenosylhomocysteine (SAH) to release adenine and the production of 5''-methylthioribose (MTR) from 5''-methylthioadenosine (MTA), also releasing adenine ( 11,  19,  28).	transcription
79148	6	335508	6	NULL	NULL	0	NULL	MTR	GP		is produced from					MTA	GP				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_13_3450_s_43	12057938	Pfs catalyzes two reactions in bacterial cells: the formation of  S-ribosylhomocysteine (SRH) from  S-adenosylhomocysteine (SAH) to release adenine and the production of 5''-methylthioribose (MTR) from 5''-methylthioadenosine (MTA), also releasing adenine ( 11,  19,  28).	transcription
79149	7	335508	6	NULL	NULL	0	NULL	MTR	GP		is					5''-methylthioribose	GP				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_13_3450_s_43	12057938	Pfs catalyzes two reactions in bacterial cells: the formation of  S-ribosylhomocysteine (SRH) from  S-adenosylhomocysteine (SAH) to release adenine and the production of 5''-methylthioribose (MTR) from 5''-methylthioadenosine (MTA), also releasing adenine ( 11,  19,  28).	transcription
79150	8	335508	6	NULL	NULL	0	NULL	MTA	GP		is					5''-methylthioadenosine	GP				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_13_3450_s_43	12057938	Pfs catalyzes two reactions in bacterial cells: the formation of  S-ribosylhomocysteine (SRH) from  S-adenosylhomocysteine (SAH) to release adenine and the production of 5''-methylthioribose (MTR) from 5''-methylthioadenosine (MTA), also releasing adenine ( 11,  19,  28).	transcription
79151	9	335508	6	NULL	NULL	0	NULL	statement 6	Process		releases					adenine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_13_3450_s_43	12057938	Pfs catalyzes two reactions in bacterial cells: the formation of  S-ribosylhomocysteine (SRH) from  S-adenosylhomocysteine (SAH) to release adenine and the production of 5''-methylthioribose (MTR) from 5''-methylthioadenosine (MTA), also releasing adenine ( 11,  19,  28).	transcription
59706	1	335508	7	NULL	NULL	0	NULL	SRH	Chemical		formed from					SAH	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_13_3450_s_43	12057938	Pfs catalyzes two reactions in bacterial cells: the formation of  S-ribosylhomocysteine (SRH) from  S-adenosylhomocysteine (SAH) to release adenine and the production of 5''-methylthioribose (MTR) from 5''-methylthioadenosine (MTA), also releasing adenine ( 11,  19,  28).	transcription
59809	2	335508	7	NULL	NULL	0	NULL	statement 1	Process		release					Adenine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_13_3450_s_43	12057938	Pfs catalyzes two reactions in bacterial cells: the formation of  S-ribosylhomocysteine (SRH) from  S-adenosylhomocysteine (SAH) to release adenine and the production of 5''-methylthioribose (MTR) from 5''-methylthioadenosine (MTA), also releasing adenine ( 11,  19,  28).	transcription
59810	3	335508	7	NULL	NULL	0	NULL	Pfs	Chemical		catalyze					statement 1	Process				NULL	bacterial cells	0	NULL	NULL	NULL	gw60_jbacteriol_184_13_3450_s_43	12057938	Pfs catalyzes two reactions in bacterial cells: the formation of  S-ribosylhomocysteine (SRH) from  S-adenosylhomocysteine (SAH) to release adenine and the production of 5''-methylthioribose (MTR) from 5''-methylthioadenosine (MTA), also releasing adenine ( 11,  19,  28).	transcription
59811	4	335508	7	NULL	NULL	0	NULL	MTR	Chemical		formed from					MTA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_13_3450_s_43	12057938	Pfs catalyzes two reactions in bacterial cells: the formation of  S-ribosylhomocysteine (SRH) from  S-adenosylhomocysteine (SAH) to release adenine and the production of 5''-methylthioribose (MTR) from 5''-methylthioadenosine (MTA), also releasing adenine ( 11,  19,  28).	transcription
59812	5	335508	7	NULL	NULL	0	NULL	statement 4	Process		release					Adenine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_13_3450_s_43	12057938	Pfs catalyzes two reactions in bacterial cells: the formation of  S-ribosylhomocysteine (SRH) from  S-adenosylhomocysteine (SAH) to release adenine and the production of 5''-methylthioribose (MTR) from 5''-methylthioadenosine (MTA), also releasing adenine ( 11,  19,  28).	transcription
59813	6	335508	7	NULL	NULL	0	NULL	Pfs	Chemical		catalyze					statement 5	Process				NULL	bacterial cells	0	NULL	NULL	NULL	gw60_jbacteriol_184_13_3450_s_43	12057938	Pfs catalyzes two reactions in bacterial cells: the formation of  S-ribosylhomocysteine (SRH) from  S-adenosylhomocysteine (SAH) to release adenine and the production of 5''-methylthioribose (MTR) from 5''-methylthioadenosine (MTA), also releasing adenine ( 11,  19,  28).	transcription
59814	7	335508	7	NULL	NULL	0	NULL	SRH	Chemical		is					S-ribosylhomocysteine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_13_3450_s_43	12057938	Pfs catalyzes two reactions in bacterial cells: the formation of  S-ribosylhomocysteine (SRH) from  S-adenosylhomocysteine (SAH) to release adenine and the production of 5''-methylthioribose (MTR) from 5''-methylthioadenosine (MTA), also releasing adenine ( 11,  19,  28).	transcription
59815	8	335508	7	NULL	NULL	0	NULL	SAH	Chemical		is					S-adenosylhomocysteine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_13_3450_s_43	12057938	Pfs catalyzes two reactions in bacterial cells: the formation of  S-ribosylhomocysteine (SRH) from  S-adenosylhomocysteine (SAH) to release adenine and the production of 5''-methylthioribose (MTR) from 5''-methylthioadenosine (MTA), also releasing adenine ( 11,  19,  28).	transcription
59816	9	335508	7	NULL	NULL	0	NULL	MTR	Chemical		is					5''-methylthioadenosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_13_3450_s_43	12057938	Pfs catalyzes two reactions in bacterial cells: the formation of  S-ribosylhomocysteine (SRH) from  S-adenosylhomocysteine (SAH) to release adenine and the production of 5''-methylthioribose (MTR) from 5''-methylthioadenosine (MTA), also releasing adenine ( 11,  19,  28).	transcription
79152	1	335509	6	NULL	NULL	0	NULL	palmitoyl-CoA	Chemical		inhibits					adenine nucleotide translocator	GP				NULL		0	NULL	NULL	NULL	gw70_diabetes_54_4_944_s_3	15793231	We found that 5 mumol/l palmitoyl-CoA inhibited adenine nucleotide translocator, without direct effect on other components of oxidative phosphorylation.	transcription
79153	2	335509	6	NULL	NULL	0	NULL	statement 1	Process		does not effect					oxidative phosphorylation	Process				NULL		0	NULL	NULL	NULL	gw70_diabetes_54_4_944_s_3	15793231	We found that 5 mumol/l palmitoyl-CoA inhibited adenine nucleotide translocator, without direct effect on other components of oxidative phosphorylation.	transcription
59817	1	335509	7	NULL	NULL	0	NULL	 palmitoyl-CoA	Chemical		inhibit					adenine nucleotide translocator	Chemical				NULL		0	NULL	NULL	NULL	gw70_diabetes_54_4_944_s_3	15793231	We found that 5 mumol/l palmitoyl-CoA inhibited adenine nucleotide translocator, without direct effect on other components of oxidative phosphorylation.	transcription
59818	2	335509	7	NULL	NULL	0	NULL	statement 1	Process		does not effect		directly			oxidative phosphorylation	Process	other components of			NULL		NULL	NULL	NULL	NULL	gw70_diabetes_54_4_944_s_3	15793231	We found that 5 mumol/l palmitoyl-CoA inhibited adenine nucleotide translocator, without direct effect on other components of oxidative phosphorylation.	transcription
59819	1	335510	7	NULL	NULL	0	NULL	MrgA family	GP	murine	respond to					RF-amide peptides	GP				NULL		0	NULL	NULL	NULL	gw70_brainresmolbrainres_142_1_58_s_146	16246453	In contrast, the only  ligand described for rMrgA is adenine   [1, although two members of the murine MrgA family respond to a number of RF-amide peptides    [5] and   [8.	transcription
59820	2	335510	7	NULL	NULL	0	NULL	adenine	Chemical		ligand for					rMrgA	GP				NULL		0	NULL	NULL	NULL	gw70_brainresmolbrainres_142_1_58_s_146	16246453	In contrast, the only  ligand described for rMrgA is adenine   [1, although two members of the murine MrgA family respond to a number of RF-amide peptides    [5] and   [8.	transcription
79154	1	335511	6	NULL	NULL	0	NULL	GTP/dGTP	Chemical		does not activate					Apaf-1	GP				NULL		0	NULL	NULL	NULL	gw70_nature_434_7035_926_s_109	15829969	These two hydrogen bonds are specific  for the adenine base but not the guanine, explaining why GTP/dGTP fails to activate  Apaf-1 (refs  3,  5).	transcription
59821	1	335511	7	NULL	NULL	0	NULL	GTP/dGTP	NucleicAcid		fails to activate					Apaf-1	GP				NULL		NULL	NULL	NULL	NULL	gw70_nature_434_7035_926_s_109	15829969	These two hydrogen bonds are specific  for the adenine base but not the guanine, explaining why GTP/dGTP fails to activate  Apaf-1 (refs  3,  5).	transcription
59822	1	335512	7	NULL	NULL	0	NULL	 5''-aziridine adenylate 1	Chemical		substitute for					SAM	Chemical				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_5_1644_s_18	15778434	The 5''-aziridine adenylate  1 is a substitute for SAM in the M.TaqI catalyzed alkylation of adenine within the recognition sequence d(TCGA) as depicted in  Scheme 1 (  -  ).	transcription
59823	2	335512	7	NULL	NULL	0	NULL	statement 1	Process		present in					 M.TaqI 	GP				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_5_1644_s_18	15778434	The 5''-aziridine adenylate  1 is a substitute for SAM in the M.TaqI catalyzed alkylation of adenine within the recognition sequence d(TCGA) as depicted in  Scheme 1 (  -  ).	transcription
59824	3	335512	7	NULL	NULL	0	NULL	 M.TaqI 	GP		catalyze					adenine	Chemical	alkylation of 			NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_5_1644_s_18	15778434	The 5''-aziridine adenylate  1 is a substitute for SAM in the M.TaqI catalyzed alkylation of adenine within the recognition sequence d(TCGA) as depicted in  Scheme 1 (  -  ).	transcription
59825	4	335512	7	NULL	NULL	0	NULL	statement 3	Process		occurs within									recognition sequence d(TCGA)	NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_5_1644_s_18	15778434	The 5''-aziridine adenylate  1 is a substitute for SAM in the M.TaqI catalyzed alkylation of adenine within the recognition sequence d(TCGA) as depicted in  Scheme 1 (  -  ).	transcription
79155	1	335513	6	NULL	NULL	0	NULL	PABP	GP		bind					PABP mRNA	NucleicAcid			ARS in 5''-untranslated region	NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_4	16356927	(A)-binding protein (PABP) mRNA translation involves the binding of PABP to the adenine-rich autoregulatory sequence (ARS) in the 5''-untranslated region of its own mRNA.	transcription
79156	2	335513	6	NULL	NULL	0	NULL	ARS	GP		is					adenine-rich autoregulatory sequence	GP				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_4	16356927	(A)-binding protein (PABP) mRNA translation involves the binding of PABP to the adenine-rich autoregulatory sequence (ARS) in the 5''-untranslated region of its own mRNA.	transcription
59826	1	335513	7	NULL	NULL	0	NULL	PABP	GP		bind									ARS	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_4	16356927	(A)-binding protein (PABP) mRNA translation involves the binding of PABP to the adenine-rich autoregulatory sequence (ARS) in the 5''-untranslated region of its own mRNA.	transcription
59827	2	335513	7	NULL	NULL	0	NULL	statement 1	Process		occur in the					PABP mRNA	GP	5''-untranslated region of			NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_4	16356927	(A)-binding protein (PABP) mRNA translation involves the binding of PABP to the adenine-rich autoregulatory sequence (ARS) in the 5''-untranslated region of its own mRNA.	transcription
59828	3	335513	7	NULL	NULL	0	NULL	PABP mRNA	GP	translation of	involves					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_22_7074_s_4	16356927	(A)-binding protein (PABP) mRNA translation involves the binding of PABP to the adenine-rich autoregulatory sequence (ARS) in the 5''-untranslated region of its own mRNA.	transcription
59829	1	335514	7	NULL	NULL	0	NULL	Dir.956-1	GP		changed to				5''-GGCCGC	Dir.956-1	GP			5''-GACCAC	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_6_2042_s_98	15817568	The IGS of Dir.956-1 was therefore changed from 5''-GGCCGC to 5''-GACCAC ( Figure 1) to allow correct base pairing between the IGS and the  E.coli SSU target sequence.	transcription
59830	2	335514	7	NULL	NULL	0	NULL				is a type of				 5''-GGCCGC	IGS	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_6_2042_s_98	15817568	The IGS of Dir.956-1 was therefore changed from 5''-GGCCGC to 5''-GACCAC ( Figure 1) to allow correct base pairing between the IGS and the  E.coli SSU target sequence.	transcription
59831	3	335514	7	NULL	NULL	0	NULL				is a type of				5''-GACCAC	IGS	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_6_2042_s_98	15817568	The IGS of Dir.956-1 was therefore changed from 5''-GGCCGC to 5''-GACCAC ( Figure 1) to allow correct base pairing between the IGS and the  E.coli SSU target sequence.	transcription
59832	4	335514	7	NULL	NULL	0	NULL				base pair with				IGS			E.coli		SSU target sequence	NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_33_6_2042_s_98	15817568	The IGS of Dir.956-1 was therefore changed from 5''-GGCCGC to 5''-GACCAC ( Figure 1) to allow correct base pairing between the IGS and the  E.coli SSU target sequence.	transcription
59833	5	335514	7	NULL	NULL	0	NULL	statement 1	Process		allows					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_33_6_2042_s_98	15817568	The IGS of Dir.956-1 was therefore changed from 5''-GGCCGC to 5''-GACCAC ( Figure 1) to allow correct base pairing between the IGS and the  E.coli SSU target sequence.	transcription
79024	1	335516	6	NULL	NULL	0	NULL	adenine	Chemical		activates					RyR	GP				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_130_7_1618_s_131	10928966	Analysis of the open and closed lifetime distributions confirms our understanding of the mechanisms underlying adenine activation of RyR and can be seen in  Figure 5.	transcription
59849	1	335516	7	NULL	NULL	0	NULL	adenine	Chemical		activates					RyR	GP				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_130_7_1618_s_131	10928966	Analysis of the open and closed lifetime distributions confirms our understanding of the mechanisms underlying adenine activation of RyR and can be seen in  Figure 5.	transcription
59850	1	335517	7	NULL	NULL	0	NULL	adenine	Chemical		regulates					Bas1p target genes	GP				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_23_4665_s_222	11095676	The identification of BIRD function in Bas1p allows us to propose a specific model for adenine regulation of Bas1p target genes, as illustrated in Figure  5.	transcription
59851	2	335517	7	NULL	NULL	0	NULL				identified in			BIRD function		Bas1p	GP				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_23_4665_s_222	11095676	The identification of BIRD function in Bas1p allows us to propose a specific model for adenine regulation of Bas1p target genes, as illustrated in Figure  5.	transcription
79025	1	335518	6	NULL	NULL	0	NULL	thymidine	Chemical		interacts with					adenine	Chemical				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_10_2183_s_3	12000838	The structure of 5''-ApTpApT-3'' has been shown to be stabilized by the 5-methyl group in the thymidine moiety that favorably interacts with the adenine pi-ring preceding it.	transcription
59852	1	335518	7	NULL	NULL	0	NULL	 5''-ApTpApT-3''	NucleicAcid	structure of	stabilized by					thymidine	NucleicAcid			5-methyl group in	NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_30_10_2183_s_3	12000838	The structure of 5''-ApTpApT-3'' has been shown to be stabilized by the 5-methyl group in the thymidine moiety that favorably interacts with the adenine pi-ring preceding it.	transcription
59853	2	335518	7	NULL	NULL	0	NULL	thymidine	NucleicAcid		interacts with		favorably		5-methyl group in	adenine	Chemical			pi-ring	NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_30_10_2183_s_3	12000838	The structure of 5''-ApTpApT-3'' has been shown to be stabilized by the 5-methyl group in the thymidine moiety that favorably interacts with the adenine pi-ring preceding it.	transcription
79026	1	335520	6	NULL	NULL	0	NULL	Aer energy taxis protein	GP	E.coli	bind			PAS domain		flavin adenine dinucleotide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_24_7206_s_25	11717280	It is particularly noteworthy that the PAS domain of the Aer energy taxis protein of  E. coli binds a flavin adenine dinucleotide to sense changes in cellular redox ( 5,  34).	transcription
59854	1	335520	7	NULL	NULL	0	NULL	Aer energy taxis protein	GP	E.coli	bind			PAS domain		flavin adenine dinucleotide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_24_7206_s_25	11717280	It is particularly noteworthy that the PAS domain of the Aer energy taxis protein of  E. coli binds a flavin adenine dinucleotide to sense changes in cellular redox ( 5,  34).	transcription
59855	2	335520	7	NULL	NULL	0	NULL	statement 1	Process		occurs to					cellular redox	Process	sense changes in			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_24_7206_s_25	11717280	It is particularly noteworthy that the PAS domain of the Aer energy taxis protein of  E. coli binds a flavin adenine dinucleotide to sense changes in cellular redox ( 5,  34).	transcription
79027	1	335521	6	NULL	NULL	NULL	NULL	adenine	Chemical		activates					SDH	GP				NULL	cauliflower mitochondria	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_35_32567_s_271	11350973	It has been observed previously, however, that SDH activation by adenine nucleotides in cauliflower mitochondria is negatively affected by sonication or freeze-thawing treatments ( 5).	transcription
59856	1	335521	7	NULL	NULL	0	NULL	adenine nucleotides	NucleicAcid	cauliflower mitochondria	activates					SDH	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_35_32567_s_271	11350973	It has been observed previously, however, that SDH activation by adenine nucleotides in cauliflower mitochondria is negatively affected by sonication or freeze-thawing treatments ( 5).	transcription
59857	2	335521	7	NULL	NULL	0	NULL	sonication	Process		affect		negatively			statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_35_32567_s_271	11350973	It has been observed previously, however, that SDH activation by adenine nucleotides in cauliflower mitochondria is negatively affected by sonication or freeze-thawing treatments ( 5).	transcription
59858	3	335521	7	NULL	NULL	0	NULL	freeze-thawing	Process		affect		negatively			statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_35_32567_s_271	11350973	It has been observed previously, however, that SDH activation by adenine nucleotides in cauliflower mitochondria is negatively affected by sonication or freeze-thawing treatments ( 5).	transcription
59862	4	335521	7	NULL	NULL	0	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_35_32567_s_271	11350973	It has been observed previously, however, that SDH activation by adenine nucleotides in cauliflower mitochondria is negatively affected by sonication or freeze-thawing treatments ( 5).	transcription
59859	1	335522	7	NULL	NULL	0	NULL	3'',5''-ADP	NucleicAcid		hydrogen bond with				Atoms N6 of adenosine				Asn-70		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_18_15009_s_233	11154698	Atoms N6 and N1 of the adenosine of 3'',5''-ADP form hydrogen bonds with Asn-70, and the adenine ring is engaged in stacking interactions with the imidazole of His-129.	transcription
59860	2	335522	7	NULL	NULL	0	NULL	3'',5''-ADP	NucleicAcid		hydrogen bond with				Atom N1 of the adenosine				Asn-70		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_18_15009_s_233	11154698	Atoms N6 and N1 of the adenosine of 3'',5''-ADP form hydrogen bonds with Asn-70, and the adenine ring is engaged in stacking interactions with the imidazole of His-129.	transcription
59861	3	335522	7	NULL	NULL	0	NULL	adenine ring 	Chemical		is engaged in							stacking interactions with	imidazole of His-129		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_18_15009_s_233	11154698	Atoms N6 and N1 of the adenosine of 3'',5''-ADP form hydrogen bonds with Asn-70, and the adenine ring is engaged in stacking interactions with the imidazole of His-129.	transcription
54967	1	335523	5	NULL	NULL	0	NULL	adenylyl cyclase			bind					AMP					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_26_16332_s_19	9632695	The crystal structure of adenylyl cyclase with bound 2'd3'AMP reveals the amino acid residues that interact with the adenine ring of the inhibitor ( 5).	transcription
59863	1	335523	7	NULL	NULL	0	NULL	adenylyl cyclase	GP		bind					2'd3'AMP	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_26_16332_s_19	9632695	The crystal structure of adenylyl cyclase with bound 2'd3'AMP reveals the amino acid residues that interact with the adenine ring of the inhibitor ( 5).	transcription
59864	1	335524	7	NULL	NULL	0	NULL	antisense oligonucleotide	NucleicAcid		targeted to					hTR	GP			16 nucleotides of the J2a/3 loop	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_23502_s_303	15811851	A recent study ( ) shows that an antisense oligonucleotide targeting 16 nucleotides of the J2a/3 loop of hTR, including the first three adenines of the 5''- AAACAAA3'' sequence, caused a 26% decrease in telomerase activity  in vitro and an increase in hTR-DNA telomeric sequence complex formation ( ).	transcription
59865	2	335524	7	NULL	NULL	0	NULL	statement 1	Process		include					5''- AAACAAA3'' sequence	NucleicAcid			 first three adenines of	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_25_23502_s_303	15811851	A recent study ( ) shows that an antisense oligonucleotide targeting 16 nucleotides of the J2a/3 loop of hTR, including the first three adenines of the 5''- AAACAAA3'' sequence, caused a 26% decrease in telomerase activity  in vitro and an increase in hTR-DNA telomeric sequence complex formation ( ).	transcription
59866	3	335524	7	NULL	NULL	0	NULL	statement 2	Process		decrease					telomerase	GP	activity of			NULL	in vitro	0	NULL	NULL	NULL	gw70_jbiolchem_280_25_23502_s_303	15811851	A recent study ( ) shows that an antisense oligonucleotide targeting 16 nucleotides of the J2a/3 loop of hTR, including the first three adenines of the 5''- AAACAAA3'' sequence, caused a 26% decrease in telomerase activity  in vitro and an increase in hTR-DNA telomeric sequence complex formation ( ).	transcription
59867	4	335524	7	NULL	NULL	0	NULL	hTR	GP		complex with					DNA	NucleicAcid			telomeric sequence	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_25_23502_s_303	15811851	A recent study ( ) shows that an antisense oligonucleotide targeting 16 nucleotides of the J2a/3 loop of hTR, including the first three adenines of the 5''- AAACAAA3'' sequence, caused a 26% decrease in telomerase activity  in vitro and an increase in hTR-DNA telomeric sequence complex formation ( ).	transcription
59868	5	335524	7	NULL	NULL	0	NULL	statement 2	Process		increase					statement 4	Process	formation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_25_23502_s_303	15811851	A recent study ( ) shows that an antisense oligonucleotide targeting 16 nucleotides of the J2a/3 loop of hTR, including the first three adenines of the 5''- AAACAAA3'' sequence, caused a 26% decrease in telomerase activity  in vitro and an increase in hTR-DNA telomeric sequence complex formation ( ).	transcription
59894	1	335525	7	NULL	NULL	0	NULL	5-methylcytosines	Chemical	number of	is identical in					G-d5 oligomer	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_14_4099_s_207	12853627	Since the number of 5-methylcytosines is identical in  G-d5,  G-d6 and  G-d7, and each oligomer contains one commonly positioned 5-methylcytosine, the relative arrangement of the 8-oxo-adenines and 5-methylcytosine in the 5' region of the oligomer must influence triplex stability, possibly as a consequence of different interactions between the bases in the third strand.	transcription
59895	2	335525	7	NULL	NULL	0	NULL	5-methylcytosines	Chemical	number of	is identical in					G-d6 oligomer	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_14_4099_s_207	12853627	Since the number of 5-methylcytosines is identical in  G-d5,  G-d6 and  G-d7, and each oligomer contains one commonly positioned 5-methylcytosine, the relative arrangement of the 8-oxo-adenines and 5-methylcytosine in the 5' region of the oligomer must influence triplex stability, possibly as a consequence of different interactions between the bases in the third strand.	transcription
59896	3	335525	7	NULL	NULL	0	NULL	5-methylcytosines	Chemical	number of	is identical in					G-d7 oligomer	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_31_14_4099_s_207	12853627	Since the number of 5-methylcytosines is identical in  G-d5,  G-d6 and  G-d7, and each oligomer contains one commonly positioned 5-methylcytosine, the relative arrangement of the 8-oxo-adenines and 5-methylcytosine in the 5' region of the oligomer must influence triplex stability, possibly as a consequence of different interactions between the bases in the third strand.	transcription
59897	4	335525	7	NULL	NULL	0	NULL	oligomer		relative arrangement of 	influence				8-oxo-adenines in the 5' region 	triplex 		stability of			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_14_4099_s_207	12853627	Since the number of 5-methylcytosines is identical in  G-d5,  G-d6 and  G-d7, and each oligomer contains one commonly positioned 5-methylcytosine, the relative arrangement of the 8-oxo-adenines and 5-methylcytosine in the 5' region of the oligomer must influence triplex stability, possibly as a consequence of different interactions between the bases in the third strand.	transcription
59898	5	335525	7	NULL	NULL	0	NULL	oligomer		relative arrangement of	influence				5-methylcytosine in the 5' region of 	triplex		stability of			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_31_14_4099_s_207	12853627	Since the number of 5-methylcytosines is identical in  G-d5,  G-d6 and  G-d7, and each oligomer contains one commonly positioned 5-methylcytosine, the relative arrangement of the 8-oxo-adenines and 5-methylcytosine in the 5' region of the oligomer must influence triplex stability, possibly as a consequence of different interactions between the bases in the third strand.	transcription
54968	1	335526	5	NULL	NULL	0	NULL	Po		increase of	higher level than					adenine					NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_130_7_1618_s_130	10928966	Not only does ATP increase Po to much higher levels than adenine (optimal activation =0.95 with 2 mM ATP compared with 0.24 with 5 mM adenine) but a dose-dependent increase in mean open lifetimes is observed together with the dose-dependent reduction in mean closed times.	transcription
54969	2	335526	5	NULL	NULL	0	NULL	ATP			is required for					statement 1					NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_130_7_1618_s_130	10928966	Not only does ATP increase Po to much higher levels than adenine (optimal activation =0.95 with 2 mM ATP compared with 0.24 with 5 mM adenine) but a dose-dependent increase in mean open lifetimes is observed together with the dose-dependent reduction in mean closed times.	transcription
54970	1	335527	5	NULL	NULL	0	NULL	ribosomes			is inactivated by					RIPs					NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_12_2383_s_14	10871371	It is well established that adenine added to cell-free protein synthesising systems protects ribosomes from inactivation by RIPs ( 2 -  4) and that protection results from an inhibition of the RNA- N-glycosidase reaction of the uncompetitive type, adenine binding more tightly to the enzyme - substrate complex than to the free enzyme ( 5).	transcription
54971	2	335527	5	NULL	NULL	0	NULL	adenine			protects					statement 1					NULL	cell-free protein synthesising systems	0	NULL	NULL	NULL	gw60_nucleicacidsres_28_12_2383_s_14	10871371	It is well established that adenine added to cell-free protein synthesising systems protects ribosomes from inactivation by RIPs ( 2 -  4) and that protection results from an inhibition of the RNA- N-glycosidase reaction of the uncompetitive type, adenine binding more tightly to the enzyme - substrate complex than to the free enzyme ( 5).	transcription
54972	3	335527	5	NULL	NULL	0	NULL	statement 2			results from					RNA- N-glycosidase reaction		inhibition of;;uncompetitive			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_12_2383_s_14	10871371	It is well established that adenine added to cell-free protein synthesising systems protects ribosomes from inactivation by RIPs ( 2 -  4) and that protection results from an inhibition of the RNA- N-glycosidase reaction of the uncompetitive type, adenine binding more tightly to the enzyme - substrate complex than to the free enzyme ( 5).	transcription
54973	4	335527	5	NULL	NULL	0	NULL	adenine			bind					enzyme - substrate complex					NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_12_2383_s_14	10871371	It is well established that adenine added to cell-free protein synthesising systems protects ribosomes from inactivation by RIPs ( 2 -  4) and that protection results from an inhibition of the RNA- N-glycosidase reaction of the uncompetitive type, adenine binding more tightly to the enzyme - substrate complex than to the free enzyme ( 5).	transcription
54974	5	335527	5	NULL	NULL	0	NULL	adenine			bind					enzyme		free			NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_12_2383_s_14	10871371	It is well established that adenine added to cell-free protein synthesising systems protects ribosomes from inactivation by RIPs ( 2 -  4) and that protection results from an inhibition of the RNA- N-glycosidase reaction of the uncompetitive type, adenine binding more tightly to the enzyme - substrate complex than to the free enzyme ( 5).	transcription
54975	6	335527	5	NULL	NULL	0	NULL	statement 4			tighter than					statement 5					NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_12_2383_s_14	10871371	It is well established that adenine added to cell-free protein synthesising systems protects ribosomes from inactivation by RIPs ( 2 -  4) and that protection results from an inhibition of the RNA- N-glycosidase reaction of the uncompetitive type, adenine binding more tightly to the enzyme - substrate complex than to the free enzyme ( 5).	transcription
59900	1	335527	7	NULL	NULL	0	NULL	RIPs	GP		inactivate					ribosomes	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_12_2383_s_14	10871371	It is well established that adenine added to cell-free protein synthesising systems protects ribosomes from inactivation by RIPs ( 2 -  4) and that protection results from an inhibition of the RNA- N-glycosidase reaction of the uncompetitive type, adenine binding more tightly to the enzyme - substrate complex than to the free enzyme ( 5).	transcription
59902	2	335527	7	NULL	NULL	0	NULL	adenine	Chemical		added to					cell-free protein synthesising systems	Cell				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_12_2383_s_14	10871371	It is well established that adenine added to cell-free protein synthesising systems protects ribosomes from inactivation by RIPs ( 2 -  4) and that protection results from an inhibition of the RNA- N-glycosidase reaction of the uncompetitive type, adenine binding more tightly to the enzyme - substrate complex than to the free enzyme ( 5).	transcription
59903	3	335527	7	NULL	NULL	0	NULL	statement 2	Process		protects					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_12_2383_s_14	10871371	It is well established that adenine added to cell-free protein synthesising systems protects ribosomes from inactivation by RIPs ( 2 -  4) and that protection results from an inhibition of the RNA- N-glycosidase reaction of the uncompetitive type, adenine binding more tightly to the enzyme - substrate complex than to the free enzyme ( 5).	transcription
59905	4	335527	7	NULL	NULL	0	NULL	statement 3	Process		results from					RNA- N-glycosidase reaction	Process	uncompetitive inhibition of			NULL		NULL	NULL	NULL	NULL	gw60_nucleicacidsres_28_12_2383_s_14	10871371	It is well established that adenine added to cell-free protein synthesising systems protects ribosomes from inactivation by RIPs ( 2 -  4) and that protection results from an inhibition of the RNA- N-glycosidase reaction of the uncompetitive type, adenine binding more tightly to the enzyme - substrate complex than to the free enzyme ( 5).	transcription
54976	1	335528	5	NULL	NULL	0	NULL	CFTR currents			is induced by					adenine					NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_3_606_s_8	11854441	Although adenine nucleotide-induced CFTR currents were inhibited by XAC, they were highly resistant to ADA treatment; 5 U/ml ADA was required for inhibition of adenine nucleotide-induced CFTR current, whereas 1 U/ml ADA was sufficient to abolish the Ade-induced response.	transcription
54977	2	335528	5	NULL	NULL	0	NULL	XAC			inhibits					statement 1					NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_3_606_s_8	11854441	Although adenine nucleotide-induced CFTR currents were inhibited by XAC, they were highly resistant to ADA treatment; 5 U/ml ADA was required for inhibition of adenine nucleotide-induced CFTR current, whereas 1 U/ml ADA was sufficient to abolish the Ade-induced response.	transcription
54978	3	335528	5	NULL	NULL	0	NULL	statement 1			is resistant to					ADA		treatment			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_3_606_s_8	11854441	Although adenine nucleotide-induced CFTR currents were inhibited by XAC, they were highly resistant to ADA treatment; 5 U/ml ADA was required for inhibition of adenine nucleotide-induced CFTR current, whereas 1 U/ml ADA was sufficient to abolish the Ade-induced response.	transcription
54979	4	335528	5	NULL	NULL	0	NULL	ADA		large quantity of	is required for					statement 1		inhibition of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_3_606_s_8	11854441	Although adenine nucleotide-induced CFTR currents were inhibited by XAC, they were highly resistant to ADA treatment; 5 U/ml ADA was required for inhibition of adenine nucleotide-induced CFTR current, whereas 1 U/ml ADA was sufficient to abolish the Ade-induced response.	transcription
54980	5	335528	5	NULL	NULL	0	NULL	ADA		small quantity of	abolishes					Ade-induced response					NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_3_606_s_8	11854441	Although adenine nucleotide-induced CFTR currents were inhibited by XAC, they were highly resistant to ADA treatment; 5 U/ml ADA was required for inhibition of adenine nucleotide-induced CFTR current, whereas 1 U/ml ADA was sufficient to abolish the Ade-induced response.	transcription
59906	1	335528	7	NULL	NULL	0	NULL	adenine nucleotide	Chemical		induce					CFTR current	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_3_606_s_8	11854441	Although adenine nucleotide-induced CFTR currents were inhibited by XAC, they were highly resistant to ADA treatment; 5 U/ml ADA was required for inhibition of adenine nucleotide-induced CFTR current, whereas 1 U/ml ADA was sufficient to abolish the Ade-induced response.	transcription
59907	2	335528	7	NULL	NULL	0	NULL	XAC	Chemical		inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_3_606_s_8	11854441	Although adenine nucleotide-induced CFTR currents were inhibited by XAC, they were highly resistant to ADA treatment; 5 U/ml ADA was required for inhibition of adenine nucleotide-induced CFTR current, whereas 1 U/ml ADA was sufficient to abolish the Ade-induced response.	transcription
59908	3	335528	7	NULL	NULL	0	NULL	statement 1	Process		resistant to					ADA	Chemical				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_3_606_s_8	11854441	Although adenine nucleotide-induced CFTR currents were inhibited by XAC, they were highly resistant to ADA treatment; 5 U/ml ADA was required for inhibition of adenine nucleotide-induced CFTR current, whereas 1 U/ml ADA was sufficient to abolish the Ade-induced response.	transcription
59909	4	335528	7	NULL	NULL	0	NULL	Ade	Chemical		induce					response	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_3_606_s_8	11854441	Although adenine nucleotide-induced CFTR currents were inhibited by XAC, they were highly resistant to ADA treatment; 5 U/ml ADA was required for inhibition of adenine nucleotide-induced CFTR current, whereas 1 U/ml ADA was sufficient to abolish the Ade-induced response.	transcription
59910	5	335528	7	NULL	NULL	0	NULL	ADA	Chemical		abolish					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_3_606_s_8	11854441	Although adenine nucleotide-induced CFTR currents were inhibited by XAC, they were highly resistant to ADA treatment; 5 U/ml ADA was required for inhibition of adenine nucleotide-induced CFTR current, whereas 1 U/ml ADA was sufficient to abolish the Ade-induced response.	transcription
54981	1	335529	5	NULL	NULL	0	NULL	palmitoyl-CoA			inhibits		exclusively			adenine nucleotide translocator					NULL		0	NULL	NULL	NULL	gw70_diabetes_54_4_944_s_156	15793231	Figures 4 and  5 together show that 5 mumol/l palmitoyl-CoA exclusively inhibits the adenine nucleotide translocator and has no direct effect on any other component of oxidative phosphorylation.	transcription
54982	2	335529	5	NULL	NULL	0	NULL	palmitoyl-CoA			does not effect		directly			oxidative phosphorylation		component of			NULL		0	NULL	NULL	NULL	gw70_diabetes_54_4_944_s_156	15793231	Figures 4 and  5 together show that 5 mumol/l palmitoyl-CoA exclusively inhibits the adenine nucleotide translocator and has no direct effect on any other component of oxidative phosphorylation.	transcription
59911	1	335529	7	NULL	NULL	0	NULL	palmitoyl-CoA 	Chemical		inhibits		exclusively			adenine nucleotide translocator	GP				NULL		0	NULL	NULL	NULL	gw70_diabetes_54_4_944_s_156	15793231	Figures 4 and  5 together show that 5 mumol/l palmitoyl-CoA exclusively inhibits the adenine nucleotide translocator and has no direct effect on any other component of oxidative phosphorylation.	transcription
59912	2	335529	7	NULL	NULL	0	NULL	statement 1	Process		no direct effect on					oxidative phosphorylation	Process	component of			NULL		NULL	NULL	NULL	NULL	gw70_diabetes_54_4_944_s_156	15793231	Figures 4 and  5 together show that 5 mumol/l palmitoyl-CoA exclusively inhibits the adenine nucleotide translocator and has no direct effect on any other component of oxidative phosphorylation.	transcription
54983	1	335530	5	NULL	NULL	0	NULL	AMP			is					adenosine 5 -triphosphate					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1701_1_37_s_5	15450174	In the first step, an adenosine 5 -triphosphate  (AMP) moiety is transferred from nicotinamide adenine dinucleotide (NAD+) or adenosine 5 -triphosphate (ATP) to a lysine residue at the active site of DNA  ligase, forming a phosphoamide protein-nucleotide bond.	transcription
54984	2	335530	5	NULL	NULL	0	NULL	NAD+			is					nicotinamide adenine dinucleotide					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1701_1_37_s_5	15450174	In the first step, an adenosine 5 -triphosphate  (AMP) moiety is transferred from nicotinamide adenine dinucleotide (NAD+) or adenosine 5 -triphosphate (ATP) to a lysine residue at the active site of DNA  ligase, forming a phosphoamide protein-nucleotide bond.	transcription
54985	3	335530	5	NULL	NULL	0	NULL	ATP			is					adenosine 5 -triphosphate					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1701_1_37_s_5	15450174	In the first step, an adenosine 5 -triphosphate  (AMP) moiety is transferred from nicotinamide adenine dinucleotide (NAD+) or adenosine 5 -triphosphate (ATP) to a lysine residue at the active site of DNA  ligase, forming a phosphoamide protein-nucleotide bond.	transcription
54986	4	335530	5	NULL	NULL	0	NULL	AMP			is transferred from					NAD+					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1701_1_37_s_5	15450174	In the first step, an adenosine 5 -triphosphate  (AMP) moiety is transferred from nicotinamide adenine dinucleotide (NAD+) or adenosine 5 -triphosphate (ATP) to a lysine residue at the active site of DNA  ligase, forming a phosphoamide protein-nucleotide bond.	transcription
54987	5	335530	5	NULL	NULL	0	NULL	AMP			is transferred from					ATP					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1701_1_37_s_5	15450174	In the first step, an adenosine 5 -triphosphate  (AMP) moiety is transferred from nicotinamide adenine dinucleotide (NAD+) or adenosine 5 -triphosphate (ATP) to a lysine residue at the active site of DNA  ligase, forming a phosphoamide protein-nucleotide bond.	transcription
54988	6	335530	5	NULL	NULL	0	NULL	statement 4			is an alternative to					statement 5					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1701_1_37_s_5	15450174	In the first step, an adenosine 5 -triphosphate  (AMP) moiety is transferred from nicotinamide adenine dinucleotide (NAD+) or adenosine 5 -triphosphate (ATP) to a lysine residue at the active site of DNA  ligase, forming a phosphoamide protein-nucleotide bond.	transcription
54989	7	335530	5	NULL	NULL	0	NULL	AMP			is transferred to					DNA ligase			lysine residue		NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1701_1_37_s_5	15450174	In the first step, an adenosine 5 -triphosphate  (AMP) moiety is transferred from nicotinamide adenine dinucleotide (NAD+) or adenosine 5 -triphosphate (ATP) to a lysine residue at the active site of DNA  ligase, forming a phosphoamide protein-nucleotide bond.	transcription
54990	8	335530	5	NULL	NULL	0	NULL	statement 6			occurs along with					statement 7					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1701_1_37_s_5	15450174	In the first step, an adenosine 5 -triphosphate  (AMP) moiety is transferred from nicotinamide adenine dinucleotide (NAD+) or adenosine 5 -triphosphate (ATP) to a lysine residue at the active site of DNA  ligase, forming a phosphoamide protein-nucleotide bond.	transcription
54991	9	335530	5	NULL	NULL	0	NULL	DNA ligase			resides in			lysine residue		DNA ligase			active site		NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1701_1_37_s_5	15450174	In the first step, an adenosine 5 -triphosphate  (AMP) moiety is transferred from nicotinamide adenine dinucleotide (NAD+) or adenosine 5 -triphosphate (ATP) to a lysine residue at the active site of DNA  ligase, forming a phosphoamide protein-nucleotide bond.	transcription
54992	10	335530	5	NULL	NULL	0	NULL	statement 7			forms					phosphoamide bond					NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1701_1_37_s_5	15450174	In the first step, an adenosine 5 -triphosphate  (AMP) moiety is transferred from nicotinamide adenine dinucleotide (NAD+) or adenosine 5 -triphosphate (ATP) to a lysine residue at the active site of DNA  ligase, forming a phosphoamide protein-nucleotide bond.	transcription
54993	11	335530	5	NULL	NULL	0	NULL	phosphoamide bond			is a type of					protein-nucleotide bond					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1701_1_37_s_5	15450174	In the first step, an adenosine 5 -triphosphate  (AMP) moiety is transferred from nicotinamide adenine dinucleotide (NAD+) or adenosine 5 -triphosphate (ATP) to a lysine residue at the active site of DNA  ligase, forming a phosphoamide protein-nucleotide bond.	transcription
59913	1	335530	7	NULL	NULL	0	NULL	AMP	Chemical		is transferred from					NAD+	Chemical				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1701_1_37_s_5	15450174	In the first step, an adenosine 5 -triphosphate  (AMP) moiety is transferred from nicotinamide adenine dinucleotide (NAD+) or adenosine 5 -triphosphate (ATP) to a lysine residue at the active site of DNA  ligase, forming a phosphoamide protein-nucleotide bond.	transcription
59914	2	335530	7	NULL	NULL	0	NULL	AMP	Chemical		is transferred from					ATP	Chemical				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1701_1_37_s_5	15450174	In the first step, an adenosine 5 -triphosphate  (AMP) moiety is transferred from nicotinamide adenine dinucleotide (NAD+) or adenosine 5 -triphosphate (ATP) to a lysine residue at the active site of DNA  ligase, forming a phosphoamide protein-nucleotide bond.	transcription
59915	3	335530	7	NULL	NULL	0	NULL	statement 1	Process		transferred to					DNA ligase	GP		lysine residue at the active site		NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1701_1_37_s_5	15450174	In the first step, an adenosine 5 -triphosphate  (AMP) moiety is transferred from nicotinamide adenine dinucleotide (NAD+) or adenosine 5 -triphosphate (ATP) to a lysine residue at the active site of DNA  ligase, forming a phosphoamide protein-nucleotide bond.	transcription
59916	4	335530	7	NULL	NULL	0	NULL	statement 2	Process		transferred to					DNA ligase	GP		lysine residue at the active site		NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1701_1_37_s_5	15450174	In the first step, an adenosine 5 -triphosphate  (AMP) moiety is transferred from nicotinamide adenine dinucleotide (NAD+) or adenosine 5 -triphosphate (ATP) to a lysine residue at the active site of DNA  ligase, forming a phosphoamide protein-nucleotide bond.	transcription
59917	5	335530	7	NULL	NULL	0	NULL	statement 3	Process		forms					 phosphoamide protein-nucleotide bond	Process				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1701_1_37_s_5	15450174	In the first step, an adenosine 5 -triphosphate  (AMP) moiety is transferred from nicotinamide adenine dinucleotide (NAD+) or adenosine 5 -triphosphate (ATP) to a lysine residue at the active site of DNA  ligase, forming a phosphoamide protein-nucleotide bond.	transcription
59918	6	335530	7	NULL	NULL	0	NULL	statement 4	Process		forms					phosphoamide protein-nucleotide bond	Process				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1701_1_37_s_5	15450174	In the first step, an adenosine 5 -triphosphate  (AMP) moiety is transferred from nicotinamide adenine dinucleotide (NAD+) or adenosine 5 -triphosphate (ATP) to a lysine residue at the active site of DNA  ligase, forming a phosphoamide protein-nucleotide bond.	transcription
59919	7	335530	7	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1701_1_37_s_5	15450174	In the first step, an adenosine 5 -triphosphate  (AMP) moiety is transferred from nicotinamide adenine dinucleotide (NAD+) or adenosine 5 -triphosphate (ATP) to a lysine residue at the active site of DNA  ligase, forming a phosphoamide protein-nucleotide bond.	transcription
59920	8	335530	7	NULL	NULL	0	NULL	NAD+	Chemical		is					nicotinamide adenine dinucleotide	Chemical				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1701_1_37_s_5	15450174	In the first step, an adenosine 5 -triphosphate  (AMP) moiety is transferred from nicotinamide adenine dinucleotide (NAD+) or adenosine 5 -triphosphate (ATP) to a lysine residue at the active site of DNA  ligase, forming a phosphoamide protein-nucleotide bond.	transcription
59921	9	335530	7	NULL	NULL	0	NULL	ATP	Chemical		is					adenosine 5 -triphosphate	Chemical				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1701_1_37_s_5	15450174	In the first step, an adenosine 5 -triphosphate  (AMP) moiety is transferred from nicotinamide adenine dinucleotide (NAD+) or adenosine 5 -triphosphate (ATP) to a lysine residue at the active site of DNA  ligase, forming a phosphoamide protein-nucleotide bond.	transcription
60045	1	335531	7	NULL	NULL	0	NULL	adenylyl cyclases	GP		contains								adenine nucleotide binding domains		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_5_2380_s_60	8576194	Thus, the evidence supports the conclusion that  adenylyl cyclases contain distinct and interacting adenine nucleotide  binding domains for catalysis (5``-ATP) and inhibition  (2``,5``-dd-3``-ATP).	transcription
60046	2	335531	7	NULL	NULL	0	NULL	adenylyl cyclases	GP		catalyze					5``-ATP	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_5_2380_s_60	8576194	Thus, the evidence supports the conclusion that  adenylyl cyclases contain distinct and interacting adenine nucleotide  binding domains for catalysis (5``-ATP) and inhibition  (2``,5``-dd-3``-ATP).	transcription
60047	3	335531	7	NULL	NULL	0	NULL	adenylyl cyclases	GP		inhibit					2``,5``-dd-3``-ATP	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_5_2380_s_60	8576194	Thus, the evidence supports the conclusion that  adenylyl cyclases contain distinct and interacting adenine nucleotide  binding domains for catalysis (5``-ATP) and inhibition  (2``,5``-dd-3``-ATP).	transcription
54994	1	335532	5	NULL	NULL	0	NULL	DEN			stimulates					taste membranes					NULL		0	NULL	NULL	NULL	gw60_pnas_96_17_9903_s_70	10449792	As with GMP (Fig.  1 e), adenosine 5''-carboxylate, adenosine 5''-monosulfate, theophylline, adenine, adenosine, cAMP, and caffeine did not block activation of transducin by DEN-stimulated taste membranes (Fig.  2).	transcription
54995	2	335532	5	NULL	NULL	0	NULL	transducin			is activated by					statement 1					NULL		0	NULL	NULL	NULL	gw60_pnas_96_17_9903_s_70	10449792	As with GMP (Fig.  1 e), adenosine 5''-carboxylate, adenosine 5''-monosulfate, theophylline, adenine, adenosine, cAMP, and caffeine did not block activation of transducin by DEN-stimulated taste membranes (Fig.  2).	transcription
54996	3	335532	5	NULL	NULL	0	NULL	adenosine 5''-carboxylate			does not block					statement 2					NULL		0	NULL	NULL	NULL	gw60_pnas_96_17_9903_s_70	10449792	As with GMP (Fig.  1 e), adenosine 5''-carboxylate, adenosine 5''-monosulfate, theophylline, adenine, adenosine, cAMP, and caffeine did not block activation of transducin by DEN-stimulated taste membranes (Fig.  2).	transcription
54997	4	335532	5	NULL	NULL	0	NULL	adenosine 5''-monosulfate			does not block					statement 2					NULL		0	NULL	NULL	NULL	gw60_pnas_96_17_9903_s_70	10449792	As with GMP (Fig.  1 e), adenosine 5''-carboxylate, adenosine 5''-monosulfate, theophylline, adenine, adenosine, cAMP, and caffeine did not block activation of transducin by DEN-stimulated taste membranes (Fig.  2).	transcription
54998	5	335532	5	NULL	NULL	0	NULL	theophylline			does not block					statement 2					NULL		0	NULL	NULL	NULL	gw60_pnas_96_17_9903_s_70	10449792	As with GMP (Fig.  1 e), adenosine 5''-carboxylate, adenosine 5''-monosulfate, theophylline, adenine, adenosine, cAMP, and caffeine did not block activation of transducin by DEN-stimulated taste membranes (Fig.  2).	transcription
54999	6	335532	5	NULL	NULL	0	NULL	adenine			does not block					statement 2					NULL		0	NULL	NULL	NULL	gw60_pnas_96_17_9903_s_70	10449792	As with GMP (Fig.  1 e), adenosine 5''-carboxylate, adenosine 5''-monosulfate, theophylline, adenine, adenosine, cAMP, and caffeine did not block activation of transducin by DEN-stimulated taste membranes (Fig.  2).	transcription
55000	7	335532	5	NULL	NULL	0	NULL	adenosine			does not block					statement 2					NULL		0	NULL	NULL	NULL	gw60_pnas_96_17_9903_s_70	10449792	As with GMP (Fig.  1 e), adenosine 5''-carboxylate, adenosine 5''-monosulfate, theophylline, adenine, adenosine, cAMP, and caffeine did not block activation of transducin by DEN-stimulated taste membranes (Fig.  2).	transcription
55001	8	335532	5	NULL	NULL	0	NULL	cAMP			does not block					statement 2					NULL		0	NULL	NULL	NULL	gw60_pnas_96_17_9903_s_70	10449792	As with GMP (Fig.  1 e), adenosine 5''-carboxylate, adenosine 5''-monosulfate, theophylline, adenine, adenosine, cAMP, and caffeine did not block activation of transducin by DEN-stimulated taste membranes (Fig.  2).	transcription
55002	9	335532	5	NULL	NULL	0	NULL	caffeine			does not block					statement 2					NULL		0	NULL	NULL	NULL	gw60_pnas_96_17_9903_s_70	10449792	As with GMP (Fig.  1 e), adenosine 5''-carboxylate, adenosine 5''-monosulfate, theophylline, adenine, adenosine, cAMP, and caffeine did not block activation of transducin by DEN-stimulated taste membranes (Fig.  2).	transcription
59922	1	335532	7	NULL	NULL	0	NULL	DEN	Chemical		stimulate					taste membranes	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_96_17_9903_s_70	10449792	As with GMP (Fig.  1 e), adenosine 5''-carboxylate, adenosine 5''-monosulfate, theophylline, adenine, adenosine, cAMP, and caffeine did not block activation of transducin by DEN-stimulated taste membranes (Fig.  2).	transcription
59923	2	335532	7	NULL	NULL	0	NULL	statement 1	Process		activates					transducin	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_96_17_9903_s_70	10449792	As with GMP (Fig.  1 e), adenosine 5''-carboxylate, adenosine 5''-monosulfate, theophylline, adenine, adenosine, cAMP, and caffeine did not block activation of transducin by DEN-stimulated taste membranes (Fig.  2).	transcription
59924	3	335532	7	NULL	NULL	0	NULL	GMP	Chemical		does not block					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_96_17_9903_s_70	10449792	As with GMP (Fig.  1 e), adenosine 5''-carboxylate, adenosine 5''-monosulfate, theophylline, adenine, adenosine, cAMP, and caffeine did not block activation of transducin by DEN-stimulated taste membranes (Fig.  2).	transcription
59925	4	335532	7	NULL	NULL	0	NULL	adenosine 5''-carboxylate	Chemical		does not block					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_96_17_9903_s_70	10449792	As with GMP (Fig.  1 e), adenosine 5''-carboxylate, adenosine 5''-monosulfate, theophylline, adenine, adenosine, cAMP, and caffeine did not block activation of transducin by DEN-stimulated taste membranes (Fig.  2).	transcription
59926	5	335532	7	NULL	NULL	0	NULL	adenosine 5''-monosulfate	Chemical		does not block					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_96_17_9903_s_70	10449792	As with GMP (Fig.  1 e), adenosine 5''-carboxylate, adenosine 5''-monosulfate, theophylline, adenine, adenosine, cAMP, and caffeine did not block activation of transducin by DEN-stimulated taste membranes (Fig.  2).	transcription
59927	6	335532	7	NULL	NULL	0	NULL	theophylline	Chemical		does not block					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_96_17_9903_s_70	10449792	As with GMP (Fig.  1 e), adenosine 5''-carboxylate, adenosine 5''-monosulfate, theophylline, adenine, adenosine, cAMP, and caffeine did not block activation of transducin by DEN-stimulated taste membranes (Fig.  2).	transcription
59928	7	335532	7	NULL	NULL	0	NULL	adenine	Chemical		does not block					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_96_17_9903_s_70	10449792	As with GMP (Fig.  1 e), adenosine 5''-carboxylate, adenosine 5''-monosulfate, theophylline, adenine, adenosine, cAMP, and caffeine did not block activation of transducin by DEN-stimulated taste membranes (Fig.  2).	transcription
59929	8	335532	7	NULL	NULL	0	NULL	adenosine	Chemical		does not block					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_96_17_9903_s_70	10449792	As with GMP (Fig.  1 e), adenosine 5''-carboxylate, adenosine 5''-monosulfate, theophylline, adenine, adenosine, cAMP, and caffeine did not block activation of transducin by DEN-stimulated taste membranes (Fig.  2).	transcription
59930	9	335532	7	NULL	NULL	0	NULL	 cAMP	Chemical		does not block					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_96_17_9903_s_70	10449792	As with GMP (Fig.  1 e), adenosine 5''-carboxylate, adenosine 5''-monosulfate, theophylline, adenine, adenosine, cAMP, and caffeine did not block activation of transducin by DEN-stimulated taste membranes (Fig.  2).	transcription
59931	10	335532	7	NULL	NULL	0	NULL	caffeine	Chemical		does not block					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_96_17_9903_s_70	10449792	As with GMP (Fig.  1 e), adenosine 5''-carboxylate, adenosine 5''-monosulfate, theophylline, adenine, adenosine, cAMP, and caffeine did not block activation of transducin by DEN-stimulated taste membranes (Fig.  2).	transcription
55003	1	335533	5	NULL	NULL	0	NULL	NAD			is incorporated into					GAPDH					NULL		0	NULL	NULL	NULL	gw60_infectimmun_67_1_259_s_109	9864224	To determine whether the residual ADP-ribosylation reflected the addition of ADP-ribose to the proteins or the covalent attachment of NAD as was observed for the nitroprusside-stimulated incorporation of [32]NAD into GAPDH ( 16), V53D and Y104K were activated with trypsin and incubated with ARF, DTT, and either [ adenine-14]NAD or [ nicotinamide-14]NAD (Fig.  5).	transcription
55004	2	335533	5	NULL	NULL	0	NULL	nitroprusside			stimulates					statement 1					NULL		0	NULL	NULL	NULL	gw60_infectimmun_67_1_259_s_109	9864224	To determine whether the residual ADP-ribosylation reflected the addition of ADP-ribose to the proteins or the covalent attachment of NAD as was observed for the nitroprusside-stimulated incorporation of [32]NAD into GAPDH ( 16), V53D and Y104K were activated with trypsin and incubated with ARF, DTT, and either [ adenine-14]NAD or [ nicotinamide-14]NAD (Fig.  5).	transcription
59932	1	335533	7	NULL	NULL	0	NULL	NAD	Chemical		incorporated into					GAPDH	GP				NULL		0	NULL	NULL	NULL	gw60_infectimmun_67_1_259_s_109	9864224	To determine whether the residual ADP-ribosylation reflected the addition of ADP-ribose to the proteins or the covalent attachment of NAD as was observed for the nitroprusside-stimulated incorporation of [32]NAD into GAPDH ( 16), V53D and Y104K were activated with trypsin and incubated with ARF, DTT, and either [ adenine-14]NAD or [ nicotinamide-14]NAD (Fig.  5).	transcription
59933	2	335533	7	NULL	NULL	0	NULL	nitroprusside	Chemical		stimulate					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_infectimmun_67_1_259_s_109	9864224	To determine whether the residual ADP-ribosylation reflected the addition of ADP-ribose to the proteins or the covalent attachment of NAD as was observed for the nitroprusside-stimulated incorporation of [32]NAD into GAPDH ( 16), V53D and Y104K were activated with trypsin and incubated with ARF, DTT, and either [ adenine-14]NAD or [ nicotinamide-14]NAD (Fig.  5).	transcription
59934	3	335533	7	NULL	NULL	0	NULL	trypsin	GP		activates								V53D		NULL		0	NULL	NULL	NULL	gw60_infectimmun_67_1_259_s_109	9864224	To determine whether the residual ADP-ribosylation reflected the addition of ADP-ribose to the proteins or the covalent attachment of NAD as was observed for the nitroprusside-stimulated incorporation of [32]NAD into GAPDH ( 16), V53D and Y104K were activated with trypsin and incubated with ARF, DTT, and either [ adenine-14]NAD or [ nicotinamide-14]NAD (Fig.  5).	transcription
59935	4	335533	7	NULL	NULL	0	NULL	trypsin	GP		activates								Y104K		NULL		0	NULL	NULL	NULL	gw60_infectimmun_67_1_259_s_109	9864224	To determine whether the residual ADP-ribosylation reflected the addition of ADP-ribose to the proteins or the covalent attachment of NAD as was observed for the nitroprusside-stimulated incorporation of [32]NAD into GAPDH ( 16), V53D and Y104K were activated with trypsin and incubated with ARF, DTT, and either [ adenine-14]NAD or [ nicotinamide-14]NAD (Fig.  5).	transcription
55005	1	335534	5	NULL	NULL	0	NULL	Slr1134			hydrolyze					ADP-ribose					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_14_4984_s_117	15995214	Sll1054 was also highly specific for ADP-ribose but it had low activity for adenosine(5'')-tetraphospho-(5'')-adenosine (Ap4A), adenosine(5'')-pentaphospho-(5'')-adenosine (Ap5A), and NADH. Slr1134 hydrolyzed not only ADP-ribose but also NADH and flavin adenine dinucleotide (FAD).	transcription
55006	2	335534	5	NULL	NULL	0	NULL	Slr1134			hydrolyze					NADH					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_14_4984_s_117	15995214	Sll1054 was also highly specific for ADP-ribose but it had low activity for adenosine(5'')-tetraphospho-(5'')-adenosine (Ap4A), adenosine(5'')-pentaphospho-(5'')-adenosine (Ap5A), and NADH. Slr1134 hydrolyzed not only ADP-ribose but also NADH and flavin adenine dinucleotide (FAD).	transcription
55007	3	335534	5	NULL	NULL	0	NULL	Slr1134			hydrolyze					FAD					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_14_4984_s_117	15995214	Sll1054 was also highly specific for ADP-ribose but it had low activity for adenosine(5'')-tetraphospho-(5'')-adenosine (Ap4A), adenosine(5'')-pentaphospho-(5'')-adenosine (Ap5A), and NADH. Slr1134 hydrolyzed not only ADP-ribose but also NADH and flavin adenine dinucleotide (FAD).	transcription
55008	4	335534	5	NULL	NULL	0	NULL	FAD			is					flavin adenine dinucleotide 					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_14_4984_s_117	15995214	Sll1054 was also highly specific for ADP-ribose but it had low activity for adenosine(5'')-tetraphospho-(5'')-adenosine (Ap4A), adenosine(5'')-pentaphospho-(5'')-adenosine (Ap5A), and NADH. Slr1134 hydrolyzed not only ADP-ribose but also NADH and flavin adenine dinucleotide (FAD).	transcription
55009	5	335534	5	NULL	NULL	0	NULL	Sll1054			specific for		highly			ADP-ribose					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_14_4984_s_117	15995214	Sll1054 was also highly specific for ADP-ribose but it had low activity for adenosine(5'')-tetraphospho-(5'')-adenosine (Ap4A), adenosine(5'')-pentaphospho-(5'')-adenosine (Ap5A), and NADH. Slr1134 hydrolyzed not only ADP-ribose but also NADH and flavin adenine dinucleotide (FAD).	transcription
55010	6	335534	5	NULL	NULL	0	NULL	Sll1054			activity for		low			Ap4A					NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_187_14_4984_s_117	15995214	Sll1054 was also highly specific for ADP-ribose but it had low activity for adenosine(5'')-tetraphospho-(5'')-adenosine (Ap4A), adenosine(5'')-pentaphospho-(5'')-adenosine (Ap5A), and NADH. Slr1134 hydrolyzed not only ADP-ribose but also NADH and flavin adenine dinucleotide (FAD).	transcription
55011	7	335534	5	NULL	NULL	0	NULL	Ap4A			is					adenosine(5'')-tetraphospho-(5'')-adenosine					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_14_4984_s_117	15995214	Sll1054 was also highly specific for ADP-ribose but it had low activity for adenosine(5'')-tetraphospho-(5'')-adenosine (Ap4A), adenosine(5'')-pentaphospho-(5'')-adenosine (Ap5A), and NADH. Slr1134 hydrolyzed not only ADP-ribose but also NADH and flavin adenine dinucleotide (FAD).	transcription
55012	8	335534	5	NULL	NULL	0	NULL	Sll1054			activity for		low			Ap5A					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_14_4984_s_117	15995214	Sll1054 was also highly specific for ADP-ribose but it had low activity for adenosine(5'')-tetraphospho-(5'')-adenosine (Ap4A), adenosine(5'')-pentaphospho-(5'')-adenosine (Ap5A), and NADH. Slr1134 hydrolyzed not only ADP-ribose but also NADH and flavin adenine dinucleotide (FAD).	transcription
55013	9	335534	5	NULL	NULL	0	NULL	Ap5A			is					adenosine(5'')-pentaphospho-(5'')-adenosine					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_14_4984_s_117	15995214	Sll1054 was also highly specific for ADP-ribose but it had low activity for adenosine(5'')-tetraphospho-(5'')-adenosine (Ap4A), adenosine(5'')-pentaphospho-(5'')-adenosine (Ap5A), and NADH. Slr1134 hydrolyzed not only ADP-ribose but also NADH and flavin adenine dinucleotide (FAD).	transcription
55014	10	335534	5	NULL	NULL	0	NULL	Sll1054			activity for		low			NADH					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_14_4984_s_117	15995214	Sll1054 was also highly specific for ADP-ribose but it had low activity for adenosine(5'')-tetraphospho-(5'')-adenosine (Ap4A), adenosine(5'')-pentaphospho-(5'')-adenosine (Ap5A), and NADH. Slr1134 hydrolyzed not only ADP-ribose but also NADH and flavin adenine dinucleotide (FAD).	transcription
59936	1	335534	7	NULL	NULL	0	NULL	Sll1054	Chemical		specific for		highly			ADP-ribose	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_187_14_4984_s_117	15995214	Sll1054 was also highly specific for ADP-ribose but it had low activity for adenosine(5'')-tetraphospho-(5'')-adenosine (Ap4A), adenosine(5'')-pentaphospho-(5'')-adenosine (Ap5A), and NADH. Slr1134 hydrolyzed not only ADP-ribose but also NADH and flavin adenine dinucleotide (FAD).	transcription
59937	2	335534	7	NULL	NULL	0	NULL	Sll1054	Chemical		activity for		low			Ap4A	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_14_4984_s_117	15995214	Sll1054 was also highly specific for ADP-ribose but it had low activity for adenosine(5'')-tetraphospho-(5'')-adenosine (Ap4A), adenosine(5'')-pentaphospho-(5'')-adenosine (Ap5A), and NADH. Slr1134 hydrolyzed not only ADP-ribose but also NADH and flavin adenine dinucleotide (FAD).	transcription
59938	3	335534	7	NULL	NULL	0	NULL	Sll1054	Chemical		activity for		low			Ap5A	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_14_4984_s_117	15995214	Sll1054 was also highly specific for ADP-ribose but it had low activity for adenosine(5'')-tetraphospho-(5'')-adenosine (Ap4A), adenosine(5'')-pentaphospho-(5'')-adenosine (Ap5A), and NADH. Slr1134 hydrolyzed not only ADP-ribose but also NADH and flavin adenine dinucleotide (FAD).	transcription
59939	4	335534	7	NULL	NULL	0	NULL	Sll1054	Chemical		activity for		low			NADH	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_14_4984_s_117	15995214	Sll1054 was also highly specific for ADP-ribose but it had low activity for adenosine(5'')-tetraphospho-(5'')-adenosine (Ap4A), adenosine(5'')-pentaphospho-(5'')-adenosine (Ap5A), and NADH. Slr1134 hydrolyzed not only ADP-ribose but also NADH and flavin adenine dinucleotide (FAD).	transcription
59940	5	335534	7	NULL	NULL	0	NULL	Slr1134	Chemical		hydrolyze					ADP-ribose	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_14_4984_s_117	15995214	Sll1054 was also highly specific for ADP-ribose but it had low activity for adenosine(5'')-tetraphospho-(5'')-adenosine (Ap4A), adenosine(5'')-pentaphospho-(5'')-adenosine (Ap5A), and NADH. Slr1134 hydrolyzed not only ADP-ribose but also NADH and flavin adenine dinucleotide (FAD).	transcription
59941	6	335534	7	NULL	NULL	0	NULL	Slr1134	Chemical		hydrolyze					NADH	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_14_4984_s_117	15995214	Sll1054 was also highly specific for ADP-ribose but it had low activity for adenosine(5'')-tetraphospho-(5'')-adenosine (Ap4A), adenosine(5'')-pentaphospho-(5'')-adenosine (Ap5A), and NADH. Slr1134 hydrolyzed not only ADP-ribose but also NADH and flavin adenine dinucleotide (FAD).	transcription
59942	7	335534	7	NULL	NULL	0	NULL	Slr1134	Chemical		hydrolyze					FAD	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_14_4984_s_117	15995214	Sll1054 was also highly specific for ADP-ribose but it had low activity for adenosine(5'')-tetraphospho-(5'')-adenosine (Ap4A), adenosine(5'')-pentaphospho-(5'')-adenosine (Ap5A), and NADH. Slr1134 hydrolyzed not only ADP-ribose but also NADH and flavin adenine dinucleotide (FAD).	transcription
59943	8	335534	7	NULL	NULL	0	NULL	Ap4A	Chemical		is					adenosine(5'')-tetraphospho-(5'')-adenosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_14_4984_s_117	15995214	Sll1054 was also highly specific for ADP-ribose but it had low activity for adenosine(5'')-tetraphospho-(5'')-adenosine (Ap4A), adenosine(5'')-pentaphospho-(5'')-adenosine (Ap5A), and NADH. Slr1134 hydrolyzed not only ADP-ribose but also NADH and flavin adenine dinucleotide (FAD).	transcription
59944	9	335534	7	NULL	NULL	0	NULL	Ap5A	Chemical		is					adenosine(5'')-pentaphospho-(5'')-adenosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_14_4984_s_117	15995214	Sll1054 was also highly specific for ADP-ribose but it had low activity for adenosine(5'')-tetraphospho-(5'')-adenosine (Ap4A), adenosine(5'')-pentaphospho-(5'')-adenosine (Ap5A), and NADH. Slr1134 hydrolyzed not only ADP-ribose but also NADH and flavin adenine dinucleotide (FAD).	transcription
59945	10	335534	7	NULL	NULL	0	NULL	FAD	Chemical		is					flavin adenine dinucleotide	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_14_4984_s_117	15995214	Sll1054 was also highly specific for ADP-ribose but it had low activity for adenosine(5'')-tetraphospho-(5'')-adenosine (Ap4A), adenosine(5'')-pentaphospho-(5'')-adenosine (Ap5A), and NADH. Slr1134 hydrolyzed not only ADP-ribose but also NADH and flavin adenine dinucleotide (FAD).	transcription
55015	1	335535	5	NULL	NULL	0	NULL				resides within				5''-GATC-3'' sites					pac sequence	NULL		0	NULL	NULL	NULL	gw70_genetics_165_1_11_s_331	14504214	STERNBERG and COULBY 1988  ,   STERNBERG and COULBY 1990   found that cleavage of the bacteriophage P1 packaging site ( pac) was regulated by adenine methylation of seven 5''-GATC-3'' sites within the  pac sequence.	transcription
55016	2	335535	5	NULL	NULL	0	NULL	statement 1		adenine methylation of 	regulates							cleavage of;;bacteriophage P1		pac	NULL		0	NULL	NULL	NULL	gw70_genetics_165_1_11_s_331	14504214	STERNBERG and COULBY 1988  ,   STERNBERG and COULBY 1990   found that cleavage of the bacteriophage P1 packaging site ( pac) was regulated by adenine methylation of seven 5''-GATC-3'' sites within the  pac sequence.	transcription
55017	3	335535	5	NULL	NULL	0	NULL	pac			is					packaging site					NULL		0	NULL	NULL	NULL	gw70_genetics_165_1_11_s_331	14504214	STERNBERG and COULBY 1988  ,   STERNBERG and COULBY 1990   found that cleavage of the bacteriophage P1 packaging site ( pac) was regulated by adenine methylation of seven 5''-GATC-3'' sites within the  pac sequence.	transcription
59946	1	335535	7	NULL	NULL	0	NULL			cleavage of bacteriophage	regulated by				pac site	adenine	Chemical	methylation of		seven 5''-GATC-3'' sites within the pac sequence	NULL		NULL	NULL	NULL	NULL	gw70_genetics_165_1_11_s_331	14504214	STERNBERG and COULBY 1988  ,   STERNBERG and COULBY 1990   found that cleavage of the bacteriophage P1 packaging site ( pac) was regulated by adenine methylation of seven 5''-GATC-3'' sites within the  pac sequence.	transcription
59947	2	335535	7	NULL	NULL	0	NULL				is				pac site			bacteriophage		P1 packaging site	NULL		0	NULL	NULL	NULL	gw70_genetics_165_1_11_s_331	14504214	STERNBERG and COULBY 1988  ,   STERNBERG and COULBY 1990   found that cleavage of the bacteriophage P1 packaging site ( pac) was regulated by adenine methylation of seven 5''-GATC-3'' sites within the  pac sequence.	transcription
55021	1	335536	5	NULL	NULL	0	NULL	palmitoyl-CoA			inhibits		exclusively			adenine nucleotide translocator					NULL	mitochondrial matrix	NULL	NULL	NULL	NULL	gw70_diabetes_54_4_944_s_208	15793231	Under the experimental conditions used, 5 mumol/l palmitoyl-CoA exclusively inhibited adenine nucleotide translocator, and this inhibition led to an increase in deltapsi and ATP concentration in the mitochondrial matrix.	transcription
55022	2	335536	5	NULL	NULL	0	NULL	statement 1			increases					ATP		concentration of			NULL	mitochondrial matrix	0	NULL	NULL	NULL	gw70_diabetes_54_4_944_s_208	15793231	Under the experimental conditions used, 5 mumol/l palmitoyl-CoA exclusively inhibited adenine nucleotide translocator, and this inhibition led to an increase in deltapsi and ATP concentration in the mitochondrial matrix.	transcription
59948	1	335536	7	NULL	NULL	0	NULL	 palmitoyl-CoA	Chemical		inhibit		exclusively			adenine nucleotide translocator	GP				NULL		0	NULL	NULL	NULL	gw70_diabetes_54_4_944_s_208	15793231	Under the experimental conditions used, 5 mumol/l palmitoyl-CoA exclusively inhibited adenine nucleotide translocator, and this inhibition led to an increase in deltapsi and ATP concentration in the mitochondrial matrix.	transcription
59949	2	335536	7	NULL	NULL	0	NULL	statement 1	Process		leads to					deltapsi 	Process	increase in concentration of			NULL	mitochondrial matrix	NULL	NULL	NULL	NULL	gw70_diabetes_54_4_944_s_208	15793231	Under the experimental conditions used, 5 mumol/l palmitoyl-CoA exclusively inhibited adenine nucleotide translocator, and this inhibition led to an increase in deltapsi and ATP concentration in the mitochondrial matrix.	transcription
59950	3	335536	7	NULL	NULL	0	NULL	statement 1	Process		leads to					ATP	Chemical	increase in concentration of 			NULL	mitochondrial matrix	NULL	NULL	NULL	NULL	gw70_diabetes_54_4_944_s_208	15793231	Under the experimental conditions used, 5 mumol/l palmitoyl-CoA exclusively inhibited adenine nucleotide translocator, and this inhibition led to an increase in deltapsi and ATP concentration in the mitochondrial matrix.	transcription
55023	1	335537	5	NULL	NULL	0	NULL	Transglutaminase 5			is regulated by					guanine/adenine nucleotides					NULL		0	NULL	NULL	NULL	gw70_brainresmolbrainres_135_1_122_s_258	15857675	[12] E. Candi, A. Paradisi, A. Terrinoni, V. Pietroni, S. Oddi, B. Cadot, V. Jogini, M.  Meiyappan, J. Clardy, A. Finazzi-Agro and G. Melino, Transglutaminase 5 is regulated  by guanine/adenine nucleotides,  Biochem.	transcription
59951	1	335537	7	NULL	NULL	0	NULL	Transglutaminase 5	GP		is regulated by					guanine nucleotides	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_brainresmolbrainres_135_1_122_s_258	15857675	[12] E. Candi, A. Paradisi, A. Terrinoni, V. Pietroni, S. Oddi, B. Cadot, V. Jogini, M.  Meiyappan, J. Clardy, A. Finazzi-Agro and G. Melino, Transglutaminase 5 is regulated  by guanine/adenine nucleotides,  Biochem.	transcription
59952	2	335537	7	NULL	NULL	0	NULL	Transglutaminase 5	GP		is regulated by					adenine nucleotides	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_brainresmolbrainres_135_1_122_s_258	15857675	[12] E. Candi, A. Paradisi, A. Terrinoni, V. Pietroni, S. Oddi, B. Cadot, V. Jogini, M.  Meiyappan, J. Clardy, A. Finazzi-Agro and G. Melino, Transglutaminase 5 is regulated  by guanine/adenine nucleotides,  Biochem.	transcription
55024	1	335538	5	NULL	NULL	0	NULL	methylene ADP			is an inhibitor of					ectonucleotidase		extracellular			NULL		NULL	NULL	NULL	NULL	gw70_neuropharmacology_47_3_427_s_200	15275832	Considering the possibility that endogenous adenosine was key to explain our findings  here, we interfered with the normal metabolic flux of adenine nucleotides using   , -methylene ADP, an inhibitor of the extracellular 5 -ectonucleotidase.	transcription
59953	1	335538	7	NULL	NULL	0	NULL	methylene ADP	Chemical		is an inhibitor of					5 -ectonucleotidase	GP	extracellular			NULL		0	NULL	NULL	NULL	gw70_neuropharmacology_47_3_427_s_200	15275832	Considering the possibility that endogenous adenosine was key to explain our findings  here, we interfered with the normal metabolic flux of adenine nucleotides using   , -methylene ADP, an inhibitor of the extracellular 5 -ectonucleotidase.	transcription
55025	1	335539	5	NULL	NULL	0	NULL	adenosine			inhibits					adenylyl cyclases					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_8_7253_s_17	15591060	Adenylyl cyclases are inhibited by adenosine and certain adenosine derivatives such as 2''-5''-dideoxyadenosine and 2''-deoxyadenosine 3''-monophosphate that possess intact adenine rings and are known as "`P-site"` inhibitors (  -  ).	transcription
55026	2	335539	5	NULL	NULL	0	NULL	2''-5''-dideoxyadenosine			is a derivative of					adenosine					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_8_7253_s_17	15591060	Adenylyl cyclases are inhibited by adenosine and certain adenosine derivatives such as 2''-5''-dideoxyadenosine and 2''-deoxyadenosine 3''-monophosphate that possess intact adenine rings and are known as "`P-site"` inhibitors (  -  ).	transcription
55027	3	335539	5	NULL	NULL	0	NULL	2''-deoxyadenosine 3''-monophosphate			is a derivative of					adenosine					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_8_7253_s_17	15591060	Adenylyl cyclases are inhibited by adenosine and certain adenosine derivatives such as 2''-5''-dideoxyadenosine and 2''-deoxyadenosine 3''-monophosphate that possess intact adenine rings and are known as "`P-site"` inhibitors (  -  ).	transcription
55030	4	335539	5	NULL	NULL	0	NULL	2''-5''-dideoxyadenosine			inhibits					adenylyl cyclases					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_8_7253_s_17	15591060	Adenylyl cyclases are inhibited by adenosine and certain adenosine derivatives such as 2''-5''-dideoxyadenosine and 2''-deoxyadenosine 3''-monophosphate that possess intact adenine rings and are known as "`P-site"` inhibitors (  -  ).	transcription
55031	5	335539	5	NULL	NULL	0	NULL	2''-deoxyadenosine 3''-monophosphate			inhibits					adenylyl cyclases					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_8_7253_s_17	15591060	Adenylyl cyclases are inhibited by adenosine and certain adenosine derivatives such as 2''-5''-dideoxyadenosine and 2''-deoxyadenosine 3''-monophosphate that possess intact adenine rings and are known as "`P-site"` inhibitors (  -  ).	transcription
55032	6	335539	5	NULL	NULL	0	NULL	2''-5''-dideoxyadenosine			possess								adenine rings		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_8_7253_s_17	15591060	Adenylyl cyclases are inhibited by adenosine and certain adenosine derivatives such as 2''-5''-dideoxyadenosine and 2''-deoxyadenosine 3''-monophosphate that possess intact adenine rings and are known as "`P-site"` inhibitors (  -  ).	transcription
55034	7	335539	5	NULL	NULL	0	NULL	2''-deoxyadenosine 3''-monophosphate			possess								adenine rings		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_8_7253_s_17	15591060	Adenylyl cyclases are inhibited by adenosine and certain adenosine derivatives such as 2''-5''-dideoxyadenosine and 2''-deoxyadenosine 3''-monophosphate that possess intact adenine rings and are known as "`P-site"` inhibitors (  -  ).	transcription
55038	8	335539	5	NULL	NULL	0	NULL	2''-5''-dideoxyadenosine			is known as					"`P-site"` inhibitors					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_8_7253_s_17	15591060	Adenylyl cyclases are inhibited by adenosine and certain adenosine derivatives such as 2''-5''-dideoxyadenosine and 2''-deoxyadenosine 3''-monophosphate that possess intact adenine rings and are known as "`P-site"` inhibitors (  -  ).	transcription
55040	9	335539	5	NULL	NULL	0	NULL	2''-deoxyadenosine 3''-monophosphate			is known as					"`P-site"` inhibitors					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_8_7253_s_17	15591060	Adenylyl cyclases are inhibited by adenosine and certain adenosine derivatives such as 2''-5''-dideoxyadenosine and 2''-deoxyadenosine 3''-monophosphate that possess intact adenine rings and are known as "`P-site"` inhibitors (  -  ).	transcription
59954	1	335539	7	NULL	NULL	0	NULL	adenosine	Chemical		inhibit					Adenylyl cyclases	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_8_7253_s_17	15591060	Adenylyl cyclases are inhibited by adenosine and certain adenosine derivatives such as 2''-5''-dideoxyadenosine and 2''-deoxyadenosine 3''-monophosphate that possess intact adenine rings and are known as "`P-site"` inhibitors (  -  ).	transcription
59955	2	335539	7	NULL	NULL	0	NULL	2''-5''-dideoxyadenosine	Chemical		possess					adenine rings	Chemical	intact			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_8_7253_s_17	15591060	Adenylyl cyclases are inhibited by adenosine and certain adenosine derivatives such as 2''-5''-dideoxyadenosine and 2''-deoxyadenosine 3''-monophosphate that possess intact adenine rings and are known as "`P-site"` inhibitors (  -  ).	transcription
59956	3	335539	7	NULL	NULL	0	NULL	2''-deoxyadenosine 3''-monophosphate	Chemical		possess					adenine rings	Chemical	intact			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_8_7253_s_17	15591060	Adenylyl cyclases are inhibited by adenosine and certain adenosine derivatives such as 2''-5''-dideoxyadenosine and 2''-deoxyadenosine 3''-monophosphate that possess intact adenine rings and are known as "`P-site"` inhibitors (  -  ).	transcription
59957	4	335539	7	NULL	NULL	0	NULL	2''-5''-dideoxyadenosine	Chemical		is an inhibitor of								"`P-site"		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_8_7253_s_17	15591060	Adenylyl cyclases are inhibited by adenosine and certain adenosine derivatives such as 2''-5''-dideoxyadenosine and 2''-deoxyadenosine 3''-monophosphate that possess intact adenine rings and are known as "`P-site"` inhibitors (  -  ).	transcription
59958	5	335539	7	NULL	NULL	0	NULL	2''-deoxyadenosine 3''-monophosphate	Chemical		is an inhibitor of								"`P-site"		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_8_7253_s_17	15591060	Adenylyl cyclases are inhibited by adenosine and certain adenosine derivatives such as 2''-5''-dideoxyadenosine and 2''-deoxyadenosine 3''-monophosphate that possess intact adenine rings and are known as "`P-site"` inhibitors (  -  ).	transcription
59959	6	335539	7	NULL	NULL	0	NULL	2''-5''-dideoxyadenosine	Chemical		is a type of					adenosine derivative	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_8_7253_s_17	15591060	Adenylyl cyclases are inhibited by adenosine and certain adenosine derivatives such as 2''-5''-dideoxyadenosine and 2''-deoxyadenosine 3''-monophosphate that possess intact adenine rings and are known as "`P-site"` inhibitors (  -  ).	transcription
59960	7	335539	7	NULL	NULL	0	NULL	2''-deoxyadenosine 3''-monophosphate	Chemical		is a type of					adenosine derivative	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_8_7253_s_17	15591060	Adenylyl cyclases are inhibited by adenosine and certain adenosine derivatives such as 2''-5''-dideoxyadenosine and 2''-deoxyadenosine 3''-monophosphate that possess intact adenine rings and are known as "`P-site"` inhibitors (  -  ).	transcription
55041	1	335540	5	NULL	NULL	0	NULL	fat		inguinal	contains					ATP		enhanced turnover of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_42_31894_s_266	16914547	Up-regulation of the adenine nucleotide translocator (ANT2) also indicates that inguinal fat has an enhanced turnover of ATP as expected for a more thermogenically active tissue ( Table 5).	transcription
55042	2	335540	5	NULL	NULL	0	NULL	ANT2			is					adenine nucleotide translocator					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_42_31894_s_266	16914547	Up-regulation of the adenine nucleotide translocator (ANT2) also indicates that inguinal fat has an enhanced turnover of ATP as expected for a more thermogenically active tissue ( Table 5).	transcription
55043	3	335540	5	NULL	NULL	0	NULL	ANT2		upregulation of	indicates					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_42_31894_s_266	16914547	Up-regulation of the adenine nucleotide translocator (ANT2) also indicates that inguinal fat has an enhanced turnover of ATP as expected for a more thermogenically active tissue ( Table 5).	transcription
59961	1	335540	7	NULL	NULL	0	NULL	ANT2	GP	Up-regulation of	indicates					ATP	Chemical	enhanced turnover of;;inguinal fat			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_42_31894_s_266	16914547	Up-regulation of the adenine nucleotide translocator (ANT2) also indicates that inguinal fat has an enhanced turnover of ATP as expected for a more thermogenically active tissue ( Table 5).	transcription
59962	2	335540	7	NULL	NULL	0	NULL	statement 1	Process		occur in					 tissue	OrganismPart	thermogenically active			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_42_31894_s_266	16914547	Up-regulation of the adenine nucleotide translocator (ANT2) also indicates that inguinal fat has an enhanced turnover of ATP as expected for a more thermogenically active tissue ( Table 5).	transcription
59963	3	335540	7	NULL	NULL	0	NULL	ANT2	GP		is					adenine nucleotide translocator	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_42_31894_s_266	16914547	Up-regulation of the adenine nucleotide translocator (ANT2) also indicates that inguinal fat has an enhanced turnover of ATP as expected for a more thermogenically active tissue ( Table 5).	transcription
55046	1	335541	5	NULL	NULL	0	NULL	EHNA			is					erythro-9-(2-hydroxy-3-nonyl)adenine hydrochloride					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_27_24888_s_136	12707258	Inhibitor of adenosine deaminase  erythro-9-(2-hydroxy-3-nonyl)adenine hydrochloride (EHNA) blocked further  conversion of adenosine in the experiments with HUVEC, either alone ( lane  3) or in combination with lymphocytes ( lane 5).	transcription
55047	2	335541	5	NULL	NULL	0	NULL	EHNA			is an inhibitor of					adenosine deaminase					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_27_24888_s_136	12707258	Inhibitor of adenosine deaminase  erythro-9-(2-hydroxy-3-nonyl)adenine hydrochloride (EHNA) blocked further  conversion of adenosine in the experiments with HUVEC, either alone ( lane  3) or in combination with lymphocytes ( lane 5).	transcription
55048	3	335541	5	NULL	NULL	0	NULL	EHNA			blocks					adenosine		further conversion of			NULL	HUVEC	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_27_24888_s_136	12707258	Inhibitor of adenosine deaminase  erythro-9-(2-hydroxy-3-nonyl)adenine hydrochloride (EHNA) blocked further  conversion of adenosine in the experiments with HUVEC, either alone ( lane  3) or in combination with lymphocytes ( lane 5).	transcription
55049	4	335541	5	NULL	NULL	0	NULL	EHNA			blocks					adenosine		further conversion of			NULL	HUVEC in combination with lymphocytes	0	NULL	NULL	NULL	gw70_jbiolchem_278_27_24888_s_136	12707258	Inhibitor of adenosine deaminase  erythro-9-(2-hydroxy-3-nonyl)adenine hydrochloride (EHNA) blocked further  conversion of adenosine in the experiments with HUVEC, either alone ( lane  3) or in combination with lymphocytes ( lane 5).	transcription
55050	5	335541	5	NULL	NULL	0	NULL	statement 3			is an alternative to					statement 4					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_27_24888_s_136	12707258	Inhibitor of adenosine deaminase  erythro-9-(2-hydroxy-3-nonyl)adenine hydrochloride (EHNA) blocked further  conversion of adenosine in the experiments with HUVEC, either alone ( lane  3) or in combination with lymphocytes ( lane 5).	transcription
59964	1	335541	7	NULL	NULL	0	NULL	EHNA	Chemical		is an inhibitor of					adenosine deaminase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_27_24888_s_136	12707258	Inhibitor of adenosine deaminase  erythro-9-(2-hydroxy-3-nonyl)adenine hydrochloride (EHNA) blocked further  conversion of adenosine in the experiments with HUVEC, either alone ( lane  3) or in combination with lymphocytes ( lane 5).	transcription
59965	2	335541	7	NULL	NULL	0	NULL	EHNA	Chemical		is					erythro-9-(2-hydroxy-3-nonyl)adenine hydrochloride	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_27_24888_s_136	12707258	Inhibitor of adenosine deaminase  erythro-9-(2-hydroxy-3-nonyl)adenine hydrochloride (EHNA) blocked further  conversion of adenosine in the experiments with HUVEC, either alone ( lane  3) or in combination with lymphocytes ( lane 5).	transcription
59966	3	335541	7	NULL	NULL	0	NULL	EHNA	Chemical		blocks					adenosine	Chemical	conversion of			NULL	HUVEC	0	NULL	NULL	NULL	gw70_jbiolchem_278_27_24888_s_136	12707258	Inhibitor of adenosine deaminase  erythro-9-(2-hydroxy-3-nonyl)adenine hydrochloride (EHNA) blocked further  conversion of adenosine in the experiments with HUVEC, either alone ( lane  3) or in combination with lymphocytes ( lane 5).	transcription
59967	4	335541	7	NULL	NULL	0	NULL	EHNA	Chemical		blocks					adenosine	Chemical	conversion of			NULL	HUVEC and lymphocytes	0	NULL	NULL	NULL	gw70_jbiolchem_278_27_24888_s_136	12707258	Inhibitor of adenosine deaminase  erythro-9-(2-hydroxy-3-nonyl)adenine hydrochloride (EHNA) blocked further  conversion of adenosine in the experiments with HUVEC, either alone ( lane  3) or in combination with lymphocytes ( lane 5).	transcription
55051	1	335543	5	NULL	NULL	0	NULL	Ant1p			is a type of					novel adenine nucleotide transporter					NULL		0	NULL	NULL	NULL	gw60_embo_20_18_5049_s_152	11566870	Ant1p is a novel adenine nucleotide transporter   Upon reconstitution into liposomes, recombinant Ant1p catalyzed an active [14]ATP/ATP exchange that was completely inhibited by a mixture of pyridoxal 5''-phosphate and bathophenanthroline.	transcription
55052	2	335543	5	NULL	NULL	0	NULL	Ant1p		recombinant	catalyzes					ATP/ATP exchange		active			NULL		0	NULL	NULL	NULL	gw60_embo_20_18_5049_s_152	11566870	Ant1p is a novel adenine nucleotide transporter   Upon reconstitution into liposomes, recombinant Ant1p catalyzed an active [14]ATP/ATP exchange that was completely inhibited by a mixture of pyridoxal 5''-phosphate and bathophenanthroline.	transcription
55053	3	335543	5	NULL	NULL	0	NULL	pyridoxal 5''-phosphate			mixed with					bathophenanthroline					NULL		0	NULL	NULL	NULL	gw60_embo_20_18_5049_s_152	11566870	Ant1p is a novel adenine nucleotide transporter   Upon reconstitution into liposomes, recombinant Ant1p catalyzed an active [14]ATP/ATP exchange that was completely inhibited by a mixture of pyridoxal 5''-phosphate and bathophenanthroline.	transcription
55054	4	335543	5	NULL	NULL	0	NULL	ATP/ATP exchange		active	is inhibited by		completely			statement 3					NULL		0	NULL	NULL	NULL	gw60_embo_20_18_5049_s_152	11566870	Ant1p is a novel adenine nucleotide transporter   Upon reconstitution into liposomes, recombinant Ant1p catalyzed an active [14]ATP/ATP exchange that was completely inhibited by a mixture of pyridoxal 5''-phosphate and bathophenanthroline.	transcription
59968	1	335543	7	NULL	NULL	0	NULL	Ant1p	GP		is a type of					adenine nucleotide transporter	GP	novel			NULL		0	NULL	NULL	NULL	gw60_embo_20_18_5049_s_152	11566870	Ant1p is a novel adenine nucleotide transporter   Upon reconstitution into liposomes, recombinant Ant1p catalyzed an active [14]ATP/ATP exchange that was completely inhibited by a mixture of pyridoxal 5''-phosphate and bathophenanthroline.	transcription
59969	2	335543	7	NULL	NULL	0	NULL	Ant1p	GP		is reconstituted into					liposomes	CellComponent				NULL		0	NULL	NULL	NULL	gw60_embo_20_18_5049_s_152	11566870	Ant1p is a novel adenine nucleotide transporter   Upon reconstitution into liposomes, recombinant Ant1p catalyzed an active [14]ATP/ATP exchange that was completely inhibited by a mixture of pyridoxal 5''-phosphate and bathophenanthroline.	transcription
59970	3	335543	7	NULL	NULL	0	NULL	Ant1p	GP	recombinant	catalyze					activeATP/ATP	Chemical	exchange of			NULL		0	NULL	NULL	NULL	gw60_embo_20_18_5049_s_152	11566870	Ant1p is a novel adenine nucleotide transporter   Upon reconstitution into liposomes, recombinant Ant1p catalyzed an active [14]ATP/ATP exchange that was completely inhibited by a mixture of pyridoxal 5''-phosphate and bathophenanthroline.	transcription
59971	4	335543	7	NULL	NULL	0	NULL	pyridoxal 5''-phosphate	Chemical		mixed with					bathophenanthroline	Chemical				NULL		0	NULL	NULL	NULL	gw60_embo_20_18_5049_s_152	11566870	Ant1p is a novel adenine nucleotide transporter   Upon reconstitution into liposomes, recombinant Ant1p catalyzed an active [14]ATP/ATP exchange that was completely inhibited by a mixture of pyridoxal 5''-phosphate and bathophenanthroline.	transcription
59972	5	335543	7	NULL	NULL	0	NULL	statement 4	Process		inhibits		completely			statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_embo_20_18_5049_s_152	11566870	Ant1p is a novel adenine nucleotide transporter   Upon reconstitution into liposomes, recombinant Ant1p catalyzed an active [14]ATP/ATP exchange that was completely inhibited by a mixture of pyridoxal 5''-phosphate and bathophenanthroline.	transcription
55055	1	335544	5	NULL	NULL	0	NULL	7-chloro-4-nitrobenzo-2-oxa-1,3-diazole			is an analog of					adenine					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1465_1_17_s_70	10748245	It contains a nucleotide-binding site, and the binding of the adenine analogue 7-chloro-4-nitrobenzo-2-oxa-1,3-diazole [  32], of fluorescein 5''-isothiocyanate [  33] or of  N-ethylmaleimide [ 32 and   34] to subunit A inhibits ATP-hydrolysis activity.	transcription
55056	2	335544	5	NULL	NULL	0	NULL	7-chloro-4-nitrobenzo-2-oxa-1,3-diazole			bind								subunit A		NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1465_1_17_s_70	10748245	It contains a nucleotide-binding site, and the binding of the adenine analogue 7-chloro-4-nitrobenzo-2-oxa-1,3-diazole [  32], of fluorescein 5''-isothiocyanate [  33] or of  N-ethylmaleimide [ 32 and   34] to subunit A inhibits ATP-hydrolysis activity.	transcription
55057	3	335544	5	NULL	NULL	0	NULL	statement 1			inhibits					ATP		hydrolysis of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1465_1_17_s_70	10748245	It contains a nucleotide-binding site, and the binding of the adenine analogue 7-chloro-4-nitrobenzo-2-oxa-1,3-diazole [  32], of fluorescein 5''-isothiocyanate [  33] or of  N-ethylmaleimide [ 32 and   34] to subunit A inhibits ATP-hydrolysis activity.	transcription
55058	4	335544	5	NULL	NULL	0	NULL	fluorescein 5''-isothiocyanate			bind								subunit A		NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1465_1_17_s_70	10748245	It contains a nucleotide-binding site, and the binding of the adenine analogue 7-chloro-4-nitrobenzo-2-oxa-1,3-diazole [  32], of fluorescein 5''-isothiocyanate [  33] or of  N-ethylmaleimide [ 32 and   34] to subunit A inhibits ATP-hydrolysis activity.	transcription
55059	5	335544	5	NULL	NULL	0	NULL	statement 4			inhibits					ATP		hydrolysis of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1465_1_17_s_70	10748245	It contains a nucleotide-binding site, and the binding of the adenine analogue 7-chloro-4-nitrobenzo-2-oxa-1,3-diazole [  32], of fluorescein 5''-isothiocyanate [  33] or of  N-ethylmaleimide [ 32 and   34] to subunit A inhibits ATP-hydrolysis activity.	transcription
55060	6	335544	5	NULL	NULL	0	NULL	N-ethylmaleimide			bind								subunit A		NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1465_1_17_s_70	10748245	It contains a nucleotide-binding site, and the binding of the adenine analogue 7-chloro-4-nitrobenzo-2-oxa-1,3-diazole [  32], of fluorescein 5''-isothiocyanate [  33] or of  N-ethylmaleimide [ 32 and   34] to subunit A inhibits ATP-hydrolysis activity.	transcription
55061	7	335544	5	NULL	NULL	0	NULL	statement 6			inhibits					ATP		hydrolysis of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1465_1_17_s_70	10748245	It contains a nucleotide-binding site, and the binding of the adenine analogue 7-chloro-4-nitrobenzo-2-oxa-1,3-diazole [  32], of fluorescein 5''-isothiocyanate [  33] or of  N-ethylmaleimide [ 32 and   34] to subunit A inhibits ATP-hydrolysis activity.	transcription
55062	8	335544	5	NULL	NULL	0	NULL	statement 2			is an alternative to					statement 4					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1465_1_17_s_70	10748245	It contains a nucleotide-binding site, and the binding of the adenine analogue 7-chloro-4-nitrobenzo-2-oxa-1,3-diazole [  32], of fluorescein 5''-isothiocyanate [  33] or of  N-ethylmaleimide [ 32 and   34] to subunit A inhibits ATP-hydrolysis activity.	transcription
55063	9	335544	5	NULL	NULL	0	NULL	statement 4			is an alternative to					statement 6					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1465_1_17_s_70	10748245	It contains a nucleotide-binding site, and the binding of the adenine analogue 7-chloro-4-nitrobenzo-2-oxa-1,3-diazole [  32], of fluorescein 5''-isothiocyanate [  33] or of  N-ethylmaleimide [ 32 and   34] to subunit A inhibits ATP-hydrolysis activity.	transcription
59973	1	335544	7	NULL	NULL	0	NULL	7-chloro-4-nitrobenzo-2-oxa-1,3-diazole	Chemical		bind								subunit A		NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1465_1_17_s_70	10748245	It contains a nucleotide-binding site, and the binding of the adenine analogue 7-chloro-4-nitrobenzo-2-oxa-1,3-diazole [  32], of fluorescein 5''-isothiocyanate [  33] or of  N-ethylmaleimide [ 32 and   34] to subunit A inhibits ATP-hydrolysis activity.	transcription
59974	2	335544	7	NULL	NULL	0	NULL	fluorescein 5''-isothiocyanate	Chemical		bind								subunit A		NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1465_1_17_s_70	10748245	It contains a nucleotide-binding site, and the binding of the adenine analogue 7-chloro-4-nitrobenzo-2-oxa-1,3-diazole [  32], of fluorescein 5''-isothiocyanate [  33] or of  N-ethylmaleimide [ 32 and   34] to subunit A inhibits ATP-hydrolysis activity.	transcription
59975	3	335544	7	NULL	NULL	0	NULL	N-ethylmaleimide	Chemical		bind								subunit A		NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1465_1_17_s_70	10748245	It contains a nucleotide-binding site, and the binding of the adenine analogue 7-chloro-4-nitrobenzo-2-oxa-1,3-diazole [  32], of fluorescein 5''-isothiocyanate [  33] or of  N-ethylmaleimide [ 32 and   34] to subunit A inhibits ATP-hydrolysis activity.	transcription
59976	4	335544	7	NULL	NULL	0	NULL	statement 1	Process		inhibit					ATP-hydrolysis activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1465_1_17_s_70	10748245	It contains a nucleotide-binding site, and the binding of the adenine analogue 7-chloro-4-nitrobenzo-2-oxa-1,3-diazole [  32], of fluorescein 5''-isothiocyanate [  33] or of  N-ethylmaleimide [ 32 and   34] to subunit A inhibits ATP-hydrolysis activity.	transcription
59977	5	335544	7	NULL	NULL	0	NULL	statement 2	Process		inhibit					ATP-hydrolysis activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1465_1_17_s_70	10748245	It contains a nucleotide-binding site, and the binding of the adenine analogue 7-chloro-4-nitrobenzo-2-oxa-1,3-diazole [  32], of fluorescein 5''-isothiocyanate [  33] or of  N-ethylmaleimide [ 32 and   34] to subunit A inhibits ATP-hydrolysis activity.	transcription
59978	6	335544	7	NULL	NULL	0	NULL	statement 3	Process		inhibit					ATP-hydrolysis activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1465_1_17_s_70	10748245	It contains a nucleotide-binding site, and the binding of the adenine analogue 7-chloro-4-nitrobenzo-2-oxa-1,3-diazole [  32], of fluorescein 5''-isothiocyanate [  33] or of  N-ethylmaleimide [ 32 and   34] to subunit A inhibits ATP-hydrolysis activity.	transcription
59979	7	335544	7	NULL	NULL	0	NULL	7-chloro-4-nitrobenzo-2-oxa-1,3-diazole	Chemical		is an analogue of					adenine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1465_1_17_s_70	10748245	It contains a nucleotide-binding site, and the binding of the adenine analogue 7-chloro-4-nitrobenzo-2-oxa-1,3-diazole [  32], of fluorescein 5''-isothiocyanate [  33] or of  N-ethylmaleimide [ 32 and   34] to subunit A inhibits ATP-hydrolysis activity.	transcription
59980	8	335544	7	NULL	NULL	0	NULL	fluorescein 5''-isothiocyanate	Chemical		is an analogue of					adenine	Chemical				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1465_1_17_s_70	10748245	It contains a nucleotide-binding site, and the binding of the adenine analogue 7-chloro-4-nitrobenzo-2-oxa-1,3-diazole [  32], of fluorescein 5''-isothiocyanate [  33] or of  N-ethylmaleimide [ 32 and   34] to subunit A inhibits ATP-hydrolysis activity.	transcription
59981	9	335544	7	NULL	NULL	0	NULL	N-ethylmaleimide	Chemical		is an analogue of					adenine	Chemical				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1465_1_17_s_70	10748245	It contains a nucleotide-binding site, and the binding of the adenine analogue 7-chloro-4-nitrobenzo-2-oxa-1,3-diazole [  32], of fluorescein 5''-isothiocyanate [  33] or of  N-ethylmaleimide [ 32 and   34] to subunit A inhibits ATP-hydrolysis activity.	transcription
55064	1	335546	5	NULL	NULL	0	NULL	profilin		low concentrations of	increases					adenine nucleotide		rate of;;exchange of			NULL	actin monomers	0	NULL	NULL	NULL	gw60_currbiol_4_5_465_s_37	7922367	This effect may be further enhanced by a second property of profilin -- its ability at low concentrations to increase the rate of adenine nucleotide exchange (replacement of ADP by ATP) on actin monomers  [5  .	transcription
59982	1	335546	7	NULL	NULL	0	NULL	ADP	Chemical		replaced by					ATP	Chemical				NULL		0	NULL	NULL	NULL	gw60_currbiol_4_5_465_s_37	7922367	This effect may be further enhanced by a second property of profilin -- its ability at low concentrations to increase the rate of adenine nucleotide exchange (replacement of ADP by ATP) on actin monomers  [5  .	transcription
59983	2	335546	7	NULL	NULL	0	NULL	statement 1			occur on					actin monomers					NULL		0	NULL	NULL	NULL	gw60_currbiol_4_5_465_s_37	7922367	This effect may be further enhanced by a second property of profilin -- its ability at low concentrations to increase the rate of adenine nucleotide exchange (replacement of ADP by ATP) on actin monomers  [5  .	transcription
59984	3	335546	7	NULL	NULL	0	NULL	profilin	Chemical		increase					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_currbiol_4_5_465_s_37	7922367	This effect may be further enhanced by a second property of profilin -- its ability at low concentrations to increase the rate of adenine nucleotide exchange (replacement of ADP by ATP) on actin monomers  [5  .	transcription
55065	1	335547	5	NULL	NULL	0	NULL	ecto-5''-nucleotidase inhibitor			effects		may			adenosine		production of			NULL	canine coronary arteries	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_12_2298_s_50	7489256	Protocol 2: Effect of an Ecto-5''-Nucleotidase Inhibitor on Adenosine Production in Canine Coronary Arteries   Adenosine can be produced intracellularly by cytosolic 5''-nucleotidase and by  S-adenosylhomocysteine, and extracellularly by ecto-5''-nucleotidase acting on released adenine nucleotides.	transcription
59985	1	335547	7	NULL	NULL	0	NULL	Adenosine	Chemical		produced by					  5''-nucleotidase	GP	cytosolic			NULL	intracellular;;Canine Coronary Arteries	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_12_2298_s_50	7489256	Protocol 2: Effect of an Ecto-5''-Nucleotidase Inhibitor on Adenosine Production in Canine Coronary Arteries   Adenosine can be produced intracellularly by cytosolic 5''-nucleotidase and by  S-adenosylhomocysteine, and extracellularly by ecto-5''-nucleotidase acting on released adenine nucleotides.	transcription
59986	2	335547	7	NULL	NULL	0	NULL	Adenosine	Chemical		produced by					S-adenosylhomocysteine	Chemical				NULL	intracellular;;Canine Coronary Arteries	NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_12_2298_s_50	7489256	Protocol 2: Effect of an Ecto-5''-Nucleotidase Inhibitor on Adenosine Production in Canine Coronary Arteries   Adenosine can be produced intracellularly by cytosolic 5''-nucleotidase and by  S-adenosylhomocysteine, and extracellularly by ecto-5''-nucleotidase acting on released adenine nucleotides.	transcription
59987	3	335547	7	NULL	NULL	0	NULL	statement 1	Process		occur simulataneous with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_12_2298_s_50	7489256	Protocol 2: Effect of an Ecto-5''-Nucleotidase Inhibitor on Adenosine Production in Canine Coronary Arteries   Adenosine can be produced intracellularly by cytosolic 5''-nucleotidase and by  S-adenosylhomocysteine, and extracellularly by ecto-5''-nucleotidase acting on released adenine nucleotides.	transcription
59988	4	335547	7	NULL	NULL	0	NULL	Adenosine	Chemical		produced by					ecto-5''-nucleotidase	GP				NULL	extracellular	0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_12_2298_s_50	7489256	Protocol 2: Effect of an Ecto-5''-Nucleotidase Inhibitor on Adenosine Production in Canine Coronary Arteries   Adenosine can be produced intracellularly by cytosolic 5''-nucleotidase and by  S-adenosylhomocysteine, and extracellularly by ecto-5''-nucleotidase acting on released adenine nucleotides.	transcription
59989	5	335547	7	NULL	NULL	0	NULL	ecto-5''-nucleotidase	GP		act on					adenine nucleotides		released			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_15_12_2298_s_50	7489256	Protocol 2: Effect of an Ecto-5''-Nucleotidase Inhibitor on Adenosine Production in Canine Coronary Arteries   Adenosine can be produced intracellularly by cytosolic 5''-nucleotidase and by  S-adenosylhomocysteine, and extracellularly by ecto-5''-nucleotidase acting on released adenine nucleotides.	transcription
55066	1	335550	5	NULL	NULL	0	NULL	Pfu			is a type of					polymerase					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_11_2914_s_69	12003931	The 3''-5' exonuclease activity of  Pfu polymerase removes nucleotide residues from both 3' ends of the PCR product and stops on the first adenine residue because of the dATP present in the reaction.	transcription
55067	2	335550	5	NULL	NULL	0	NULL	nucleotide residues			removed from					PCR product				3' ends	NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_11_2914_s_69	12003931	The 3''-5' exonuclease activity of  Pfu polymerase removes nucleotide residues from both 3' ends of the PCR product and stops on the first adenine residue because of the dATP present in the reaction.	transcription
55068	3	335550	5	NULL	NULL	0	NULL	statement 2			stops at					adenine residue					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_11_2914_s_69	12003931	The 3''-5' exonuclease activity of  Pfu polymerase removes nucleotide residues from both 3' ends of the PCR product and stops on the first adenine residue because of the dATP present in the reaction.	transcription
55069	4	335550	5	NULL	NULL	0	NULL	statement 3			because of					dATP		presence of			NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_11_2914_s_69	12003931	The 3''-5' exonuclease activity of  Pfu polymerase removes nucleotide residues from both 3' ends of the PCR product and stops on the first adenine residue because of the dATP present in the reaction.	transcription
55070	5	335550	5	NULL	NULL	0	NULL	Pfu		3''-5' exonuclease activity of	is required for					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_11_2914_s_69	12003931	The 3''-5' exonuclease activity of  Pfu polymerase removes nucleotide residues from both 3' ends of the PCR product and stops on the first adenine residue because of the dATP present in the reaction.	transcription
59990	1	335550	7	NULL	NULL	0	NULL	Pfu polymerase	GP		possess					3''-5' exonuclease activity	Process				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_11_2914_s_69	12003931	The 3''-5' exonuclease activity of  Pfu polymerase removes nucleotide residues from both 3' ends of the PCR product and stops on the first adenine residue because of the dATP present in the reaction.	transcription
59991	2	335550	7	NULL	NULL	0	NULL	statement 1	Process		removes					nucleotide residues	NucleicAcid			from 3' end	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_184_11_2914_s_69	12003931	The 3''-5' exonuclease activity of  Pfu polymerase removes nucleotide residues from both 3' ends of the PCR product and stops on the first adenine residue because of the dATP present in the reaction.	transcription
59992	3	335550	7	NULL	NULL	0	NULL	statement 1	Process		stops					adenine residue	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_184_11_2914_s_69	12003931	The 3''-5' exonuclease activity of  Pfu polymerase removes nucleotide residues from both 3' ends of the PCR product and stops on the first adenine residue because of the dATP present in the reaction.	transcription
55071	1	335551	5	NULL	NULL	0	NULL	Oocytes			express					TbNBT1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_26_23502_s_119	12707261	Oocytes expressing  TbNBT1 rapidly accumulated  [3]adenine and, to a lesser extent, [3]uracil, but no  significant mediated transport of [3]adenosine or  [3]uridine was observed at pH 7.5  ( Fig. 5).	transcription
55072	2	335551	5	NULL	NULL	0	NULL	statement 1			accumulates		rapidly			adenine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_26_23502_s_119	12707261	Oocytes expressing  TbNBT1 rapidly accumulated  [3]adenine and, to a lesser extent, [3]uracil, but no  significant mediated transport of [3]adenosine or  [3]uridine was observed at pH 7.5  ( Fig. 5).	transcription
55073	3	335551	5	NULL	NULL	0	NULL	statement 1			accumulates					uracil					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_26_23502_s_119	12707261	Oocytes expressing  TbNBT1 rapidly accumulated  [3]adenine and, to a lesser extent, [3]uracil, but no  significant mediated transport of [3]adenosine or  [3]uridine was observed at pH 7.5  ( Fig. 5).	transcription
55074	4	335551	5	NULL	NULL	0	NULL	statement 3			lesser extent than					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_26_23502_s_119	12707261	Oocytes expressing  TbNBT1 rapidly accumulated  [3]adenine and, to a lesser extent, [3]uracil, but no  significant mediated transport of [3]adenosine or  [3]uridine was observed at pH 7.5  ( Fig. 5).	transcription
59993	1	335551	7	NULL	NULL	0	NULL	Oocytes	Cell		express					TbNBT1	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_26_23502_s_119	12707261	Oocytes expressing  TbNBT1 rapidly accumulated  [3]adenine and, to a lesser extent, [3]uracil, but no  significant mediated transport of [3]adenosine or  [3]uridine was observed at pH 7.5  ( Fig. 5).	transcription
59994	2	335551	7	NULL	NULL	0	NULL	statement 1	Process		accumulate		rapidly			adenine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_26_23502_s_119	12707261	Oocytes expressing  TbNBT1 rapidly accumulated  [3]adenine and, to a lesser extent, [3]uracil, but no  significant mediated transport of [3]adenosine or  [3]uridine was observed at pH 7.5  ( Fig. 5).	transcription
59995	3	335551	7	NULL	NULL	0	NULL	statement 1	Process		accumulate					Uracil	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_26_23502_s_119	12707261	Oocytes expressing  TbNBT1 rapidly accumulated  [3]adenine and, to a lesser extent, [3]uracil, but no  significant mediated transport of [3]adenosine or  [3]uridine was observed at pH 7.5  ( Fig. 5).	transcription
59996	4	335551	7	NULL	NULL	0	NULL	statement 3	Process	accumulation of	is lesser than					statement 2	Process	accumulation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_26_23502_s_119	12707261	Oocytes expressing  TbNBT1 rapidly accumulated  [3]adenine and, to a lesser extent, [3]uracil, but no  significant mediated transport of [3]adenosine or  [3]uridine was observed at pH 7.5  ( Fig. 5).	transcription
59997	5	335551	7	NULL	NULL	0	NULL	statement 1	Process		does not mediate					adenosine	Chemical	transport of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_26_23502_s_119	12707261	Oocytes expressing  TbNBT1 rapidly accumulated  [3]adenine and, to a lesser extent, [3]uracil, but no  significant mediated transport of [3]adenosine or  [3]uridine was observed at pH 7.5  ( Fig. 5).	transcription
59998	6	335551	7	NULL	NULL	0	NULL	statement 1	Process		does not mediate					uridine	Chemical	transport of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_26_23502_s_119	12707261	Oocytes expressing  TbNBT1 rapidly accumulated  [3]adenine and, to a lesser extent, [3]uracil, but no  significant mediated transport of [3]adenosine or  [3]uridine was observed at pH 7.5  ( Fig. 5).	transcription
55075	1	335552	5	NULL	NULL	0	NULL	mdr1a gene product			bind					adenine nucleotide					NULL	ZGM	0	NULL	NULL	NULL	gw60_jbiolchem_271_6_3300_s_156	8621734	As  summarized in the model in  Fig. 5, we propose that a  mdr1a  gene product in ZGM is an adenine nucleotide binding protein that  regulates both Cl   and K   conductances  in a coupled but inverse manner.	transcription
55076	2	335552	5	NULL	NULL	0	NULL	mdr1a gene product			regulates					Cl conductance					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_6_3300_s_156	8621734	As  summarized in the model in  Fig. 5, we propose that a  mdr1a  gene product in ZGM is an adenine nucleotide binding protein that  regulates both Cl   and K   conductances  in a coupled but inverse manner.	transcription
55077	3	335552	5	NULL	NULL	0	NULL	mdr1a gene product			regulates					K conductance					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_6_3300_s_156	8621734	As  summarized in the model in  Fig. 5, we propose that a  mdr1a  gene product in ZGM is an adenine nucleotide binding protein that  regulates both Cl   and K   conductances  in a coupled but inverse manner.	transcription
59999	1	335552	7	NULL	NULL	0	NULL	mdr1a gene	GP	product of	is a type of					adenine nucleotide binding protein					NULL	ZGM	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_6_3300_s_156	8621734	As  summarized in the model in  Fig. 5, we propose that a  mdr1a  gene product in ZGM is an adenine nucleotide binding protein that  regulates both Cl   and K   conductances  in a coupled but inverse manner.	transcription
60000	2	335552	7	NULL	NULL	0	NULL	mdr1a gene	GP	product of	regulates					Cl conductance	Process				NULL	ZGM	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_6_3300_s_156	8621734	As  summarized in the model in  Fig. 5, we propose that a  mdr1a  gene product in ZGM is an adenine nucleotide binding protein that  regulates both Cl   and K   conductances  in a coupled but inverse manner.	transcription
60001	3	335552	7	NULL	NULL	0	NULL	mdr1a gene	GP	product of	regulates					K conductance	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_6_3300_s_156	8621734	As  summarized in the model in  Fig. 5, we propose that a  mdr1a  gene product in ZGM is an adenine nucleotide binding protein that  regulates both Cl   and K   conductances  in a coupled but inverse manner.	transcription
60002	4	335552	7	NULL	NULL	0	NULL	statement 2	Process		coupled with					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_6_3300_s_156	8621734	As  summarized in the model in  Fig. 5, we propose that a  mdr1a  gene product in ZGM is an adenine nucleotide binding protein that  regulates both Cl   and K   conductances  in a coupled but inverse manner.	transcription
60003	5	335552	7	NULL	NULL	0	NULL	statement 2	Process		occur inversely to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_6_3300_s_156	8621734	As  summarized in the model in  Fig. 5, we propose that a  mdr1a  gene product in ZGM is an adenine nucleotide binding protein that  regulates both Cl   and K   conductances  in a coupled but inverse manner.	transcription
55078	1	335553	5	NULL	NULL	0	NULL	HAL2			encodes					3 (2 ),5 -bisphosphate nucleotidase					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_22_12859_s_177	8662738	HAL2 encodes a 3 (2 ),5 -bisphosphate nucleotidase required for recycling of adenine nucleotides in sulfate transfer reactions, and its phosphatase activity was inhibited by Li+ and to a lesser extend by Na+ ions ( 59).	transcription
55079	2	335553	5	NULL	NULL	0	NULL	HAL2			recycles					adenine nucleotides					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_22_12859_s_177	8662738	HAL2 encodes a 3 (2 ),5 -bisphosphate nucleotidase required for recycling of adenine nucleotides in sulfate transfer reactions, and its phosphatase activity was inhibited by Li+ and to a lesser extend by Na+ ions ( 59).	transcription
55080	3	335553	5	NULL	NULL	0	NULL	statement 2			occurs in					sulfate transfer reactions					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_22_12859_s_177	8662738	HAL2 encodes a 3 (2 ),5 -bisphosphate nucleotidase required for recycling of adenine nucleotides in sulfate transfer reactions, and its phosphatase activity was inhibited by Li+ and to a lesser extend by Na+ ions ( 59).	transcription
55081	4	335553	5	NULL	NULL	0	NULL	Li+ ions			inhibit					HAL2		phosphatase activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_22_12859_s_177	8662738	HAL2 encodes a 3 (2 ),5 -bisphosphate nucleotidase required for recycling of adenine nucleotides in sulfate transfer reactions, and its phosphatase activity was inhibited by Li+ and to a lesser extend by Na+ ions ( 59).	transcription
55082	5	335553	5	NULL	NULL	0	NULL	Na+ ion			inhibit					HAL2		phosphatase activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_22_12859_s_177	8662738	HAL2 encodes a 3 (2 ),5 -bisphosphate nucleotidase required for recycling of adenine nucleotides in sulfate transfer reactions, and its phosphatase activity was inhibited by Li+ and to a lesser extend by Na+ ions ( 59).	transcription
55083	6	335553	5	NULL	NULL	0	NULL	statement 5			lesser extent than					statement 4					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_22_12859_s_177	8662738	HAL2 encodes a 3 (2 ),5 -bisphosphate nucleotidase required for recycling of adenine nucleotides in sulfate transfer reactions, and its phosphatase activity was inhibited by Li+ and to a lesser extend by Na+ ions ( 59).	transcription
60004	1	335553	7	NULL	NULL	0	NULL	HAL2	GP		encode					3 (2 ),5 -bisphosphate nucleotidase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_22_12859_s_177	8662738	HAL2 encodes a 3 (2 ),5 -bisphosphate nucleotidase required for recycling of adenine nucleotides in sulfate transfer reactions, and its phosphatase activity was inhibited by Li+ and to a lesser extend by Na+ ions ( 59).	transcription
60005	2	335553	7	NULL	NULL	0	NULL	3 (2 ),5 -bisphosphate nucleotidase	GP		required for					adenine nucleotides	NucleicAcid	recycling of			NULL	sulfate transfer reactions	0	NULL	NULL	NULL	gw60_jbiolchem_271_22_12859_s_177	8662738	HAL2 encodes a 3 (2 ),5 -bisphosphate nucleotidase required for recycling of adenine nucleotides in sulfate transfer reactions, and its phosphatase activity was inhibited by Li+ and to a lesser extend by Na+ ions ( 59).	transcription
60006	3	335553	7	NULL	NULL	0	NULL	Li+ 	Chemical		inhibit					 3 (2 ),5 -bisphosphate nucleotidase	GP	phosphatase activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_22_12859_s_177	8662738	HAL2 encodes a 3 (2 ),5 -bisphosphate nucleotidase required for recycling of adenine nucleotides in sulfate transfer reactions, and its phosphatase activity was inhibited by Li+ and to a lesser extend by Na+ ions ( 59).	transcription
60007	4	335553	7	NULL	NULL	0	NULL	Na+ ions	Chemical		inhibit					3 (2 ),5 -bisphosphate nucleotidase	Chemical	phosphatase activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_22_12859_s_177	8662738	HAL2 encodes a 3 (2 ),5 -bisphosphate nucleotidase required for recycling of adenine nucleotides in sulfate transfer reactions, and its phosphatase activity was inhibited by Li+ and to a lesser extend by Na+ ions ( 59).	transcription
60008	5	335553	7	NULL	NULL	0	NULL	statement 4	Process	inhibition of	is lesser than					statement 3	Process	inhibition of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_22_12859_s_177	8662738	HAL2 encodes a 3 (2 ),5 -bisphosphate nucleotidase required for recycling of adenine nucleotides in sulfate transfer reactions, and its phosphatase activity was inhibited by Li+ and to a lesser extend by Na+ ions ( 59).	transcription
55084	1	335554	5	NULL	NULL	0	NULL	adenine group			contains								nitrogen atoms ( N1, N3, N6, N7, and N9)		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_6_3617_s_147	9920910	The adenine group contains five nitrogen atoms ( N1,  N3,  N6,  N7, and  N9) that can interact with receptor sites, whereas the ribose moiety contains three hydroxyl groups (2'', 3'', 5'') ( 8).	transcription
55085	2	335554	5	NULL	NULL	0	NULL	statement 1			interacts with								receptor sites		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_6_3617_s_147	9920910	The adenine group contains five nitrogen atoms ( N1,  N3,  N6,  N7, and  N9) that can interact with receptor sites, whereas the ribose moiety contains three hydroxyl groups (2'', 3'', 5'') ( 8).	transcription
55086	3	335554	5	NULL	NULL	0	NULL	ribose moiety			contains					hydroxyl groups					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_6_3617_s_147	9920910	The adenine group contains five nitrogen atoms ( N1,  N3,  N6,  N7, and  N9) that can interact with receptor sites, whereas the ribose moiety contains three hydroxyl groups (2'', 3'', 5'') ( 8).	transcription
55087	1	335555	5	NULL	NULL	0	NULL	AC			is					adenylyl cyclase					NULL		0	NULL	NULL	NULL	gw60_science_294_5545_1299_s_149	11701921	The stimulation of adenylyl cyclase (AC) by heterotrimeric G proteins  is the classic example for an allosteric effector interaction mediating  the conversion of ATP to the second messenger cyclic adenine  3''-5''-monophosphate (cAMP).	transcription
55088	2	335555	5	NULL	NULL	0	NULL	adenylyl cyclase			is stimulated by					heterotrimeric G proteins					NULL		0	NULL	NULL	NULL	gw60_science_294_5545_1299_s_149	11701921	The stimulation of adenylyl cyclase (AC) by heterotrimeric G proteins  is the classic example for an allosteric effector interaction mediating  the conversion of ATP to the second messenger cyclic adenine  3''-5''-monophosphate (cAMP).	transcription
55089	3	335555	5	NULL	NULL	0	NULL	statement 2			is an example of					allosteric effector interaction					NULL		0	NULL	NULL	NULL	gw60_science_294_5545_1299_s_149	11701921	The stimulation of adenylyl cyclase (AC) by heterotrimeric G proteins  is the classic example for an allosteric effector interaction mediating  the conversion of ATP to the second messenger cyclic adenine  3''-5''-monophosphate (cAMP).	transcription
55090	4	335555	5	NULL	NULL	0	NULL	ATP			is converted to					cAMP					NULL		0	NULL	NULL	NULL	gw60_science_294_5545_1299_s_149	11701921	The stimulation of adenylyl cyclase (AC) by heterotrimeric G proteins  is the classic example for an allosteric effector interaction mediating  the conversion of ATP to the second messenger cyclic adenine  3''-5''-monophosphate (cAMP).	transcription
55091	5	335555	5	NULL	NULL	0	NULL	cAMP			is					cyclic adenine 3''-5''-monophosphate					NULL		0	NULL	NULL	NULL	gw60_science_294_5545_1299_s_149	11701921	The stimulation of adenylyl cyclase (AC) by heterotrimeric G proteins  is the classic example for an allosteric effector interaction mediating  the conversion of ATP to the second messenger cyclic adenine  3''-5''-monophosphate (cAMP).	transcription
55092	6	335555	5	NULL	NULL	0	NULL	cAMP			is a type of					second messenger					NULL		0	NULL	NULL	NULL	gw60_science_294_5545_1299_s_149	11701921	The stimulation of adenylyl cyclase (AC) by heterotrimeric G proteins  is the classic example for an allosteric effector interaction mediating  the conversion of ATP to the second messenger cyclic adenine  3''-5''-monophosphate (cAMP).	transcription
55093	7	335555	5	NULL	NULL	0	NULL	statement 2			mediates					statement 4					NULL		0	NULL	NULL	NULL	gw60_science_294_5545_1299_s_149	11701921	The stimulation of adenylyl cyclase (AC) by heterotrimeric G proteins  is the classic example for an allosteric effector interaction mediating  the conversion of ATP to the second messenger cyclic adenine  3''-5''-monophosphate (cAMP).	transcription
60009	1	335555	7	NULL	NULL	0	NULL	heterotrimeric G proteins	GP		stimulate					AC	GP				NULL		0	NULL	NULL	NULL	gw60_science_294_5545_1299_s_149	11701921	The stimulation of adenylyl cyclase (AC) by heterotrimeric G proteins  is the classic example for an allosteric effector interaction mediating  the conversion of ATP to the second messenger cyclic adenine  3''-5''-monophosphate (cAMP).	transcription
60010	2	335555	7	NULL	NULL	0	NULL	statement 1	Process		is an example of					allosteric effector interaction	Process				NULL		0	NULL	NULL	NULL	gw60_science_294_5545_1299_s_149	11701921	The stimulation of adenylyl cyclase (AC) by heterotrimeric G proteins  is the classic example for an allosteric effector interaction mediating  the conversion of ATP to the second messenger cyclic adenine  3''-5''-monophosphate (cAMP).	transcription
60011	3	335555	7	NULL	NULL	0	NULL	AC	GP		is					adenylyl cyclase	GP				NULL		0	NULL	NULL	NULL	gw60_science_294_5545_1299_s_149	11701921	The stimulation of adenylyl cyclase (AC) by heterotrimeric G proteins  is the classic example for an allosteric effector interaction mediating  the conversion of ATP to the second messenger cyclic adenine  3''-5''-monophosphate (cAMP).	transcription
60012	4	335555	7	NULL	NULL	0	NULL	ATP	Chemical		converted to					cAMP	Chemical				NULL		0	NULL	NULL	NULL	gw60_science_294_5545_1299_s_149	11701921	The stimulation of adenylyl cyclase (AC) by heterotrimeric G proteins  is the classic example for an allosteric effector interaction mediating  the conversion of ATP to the second messenger cyclic adenine  3''-5''-monophosphate (cAMP).	transcription
60013	5	335555	7	NULL	NULL	0	NULL	cAMP	Chemical		is					cyclic adenine 3''-5''-monophosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_science_294_5545_1299_s_149	11701921	The stimulation of adenylyl cyclase (AC) by heterotrimeric G proteins  is the classic example for an allosteric effector interaction mediating  the conversion of ATP to the second messenger cyclic adenine  3''-5''-monophosphate (cAMP).	transcription
60014	6	335555	7	NULL	NULL	0	NULL	statement 1	Process		mediates					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_science_294_5545_1299_s_149	11701921	The stimulation of adenylyl cyclase (AC) by heterotrimeric G proteins  is the classic example for an allosteric effector interaction mediating  the conversion of ATP to the second messenger cyclic adenine  3''-5''-monophosphate (cAMP).	transcription
55094	1	335556	5	NULL	NULL	0	NULL	oligos			conatins					adenine					NULL		0	NULL	NULL	NULL	gw60_structure_4_10_1171_s_103	8939742	Competition experiments and  Kd determinations also show that Zif268 binds oligos with adenine or cytosine at these positions about 5 to 10-fold more tightly than oligos containing guanine or thymine ( [13]  ; Bryan Wang and COP, unpublished data).	transcription
55095	2	335556	5	NULL	NULL	0	NULL	oligos			contains					cytosine					NULL		0	NULL	NULL	NULL	gw60_structure_4_10_1171_s_103	8939742	Competition experiments and  Kd determinations also show that Zif268 binds oligos with adenine or cytosine at these positions about 5 to 10-fold more tightly than oligos containing guanine or thymine ( [13]  ; Bryan Wang and COP, unpublished data).	transcription
55096	3	335556	5	NULL	NULL	0	NULL	oligos			contains					guanine					NULL		0	NULL	NULL	NULL	gw60_structure_4_10_1171_s_103	8939742	Competition experiments and  Kd determinations also show that Zif268 binds oligos with adenine or cytosine at these positions about 5 to 10-fold more tightly than oligos containing guanine or thymine ( [13]  ; Bryan Wang and COP, unpublished data).	transcription
55097	4	335556	5	NULL	NULL	0	NULL	oligos			contains					thymine					NULL		0	NULL	NULL	NULL	gw60_structure_4_10_1171_s_103	8939742	Competition experiments and  Kd determinations also show that Zif268 binds oligos with adenine or cytosine at these positions about 5 to 10-fold more tightly than oligos containing guanine or thymine ( [13]  ; Bryan Wang and COP, unpublished data).	transcription
55098	5	335556	5	NULL	NULL	0	NULL	Zif268			bind					statement 1					NULL		0	NULL	NULL	NULL	gw60_structure_4_10_1171_s_103	8939742	Competition experiments and  Kd determinations also show that Zif268 binds oligos with adenine or cytosine at these positions about 5 to 10-fold more tightly than oligos containing guanine or thymine ( [13]  ; Bryan Wang and COP, unpublished data).	transcription
55099	6	335556	5	NULL	NULL	0	NULL	Zif268			bind					statement 2					NULL		0	NULL	NULL	NULL	gw60_structure_4_10_1171_s_103	8939742	Competition experiments and  Kd determinations also show that Zif268 binds oligos with adenine or cytosine at these positions about 5 to 10-fold more tightly than oligos containing guanine or thymine ( [13]  ; Bryan Wang and COP, unpublished data).	transcription
55100	7	335556	5	NULL	NULL	0	NULL	Zif268			bind					statement 3					NULL		0	NULL	NULL	NULL	gw60_structure_4_10_1171_s_103	8939742	Competition experiments and  Kd determinations also show that Zif268 binds oligos with adenine or cytosine at these positions about 5 to 10-fold more tightly than oligos containing guanine or thymine ( [13]  ; Bryan Wang and COP, unpublished data).	transcription
55101	8	335556	5	NULL	NULL	0	NULL	Zif268			bind					statement 4					NULL		0	NULL	NULL	NULL	gw60_structure_4_10_1171_s_103	8939742	Competition experiments and  Kd determinations also show that Zif268 binds oligos with adenine or cytosine at these positions about 5 to 10-fold more tightly than oligos containing guanine or thymine ( [13]  ; Bryan Wang and COP, unpublished data).	transcription
55102	9	335556	5	NULL	NULL	0	NULL	statement 5			is an alternative to					statement 6					NULL		0	NULL	NULL	NULL	gw60_structure_4_10_1171_s_103	8939742	Competition experiments and  Kd determinations also show that Zif268 binds oligos with adenine or cytosine at these positions about 5 to 10-fold more tightly than oligos containing guanine or thymine ( [13]  ; Bryan Wang and COP, unpublished data).	transcription
55103	10	335556	5	NULL	NULL	0	NULL	statement 7			is an alternative to					statement 8					NULL		0	NULL	NULL	NULL	gw60_structure_4_10_1171_s_103	8939742	Competition experiments and  Kd determinations also show that Zif268 binds oligos with adenine or cytosine at these positions about 5 to 10-fold more tightly than oligos containing guanine or thymine ( [13]  ; Bryan Wang and COP, unpublished data).	transcription
55104	11	335556	5	NULL	NULL	0	NULL	statement 9			more tightly than					statement 10					NULL		0	NULL	NULL	NULL	gw60_structure_4_10_1171_s_103	8939742	Competition experiments and  Kd determinations also show that Zif268 binds oligos with adenine or cytosine at these positions about 5 to 10-fold more tightly than oligos containing guanine or thymine ( [13]  ; Bryan Wang and COP, unpublished data).	transcription
60015	1	335556	7	NULL	NULL	0	NULL	Zif268	Chemical		bind					adenine oligos	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_structure_4_10_1171_s_103	8939742	Competition experiments and  Kd determinations also show that Zif268 binds oligos with adenine or cytosine at these positions about 5 to 10-fold more tightly than oligos containing guanine or thymine ( [13]  ; Bryan Wang and COP, unpublished data).	transcription
60016	2	335556	7	NULL	NULL	0	NULL	Zif268	Chemical		bind					cytosine oligos	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_structure_4_10_1171_s_103	8939742	Competition experiments and  Kd determinations also show that Zif268 binds oligos with adenine or cytosine at these positions about 5 to 10-fold more tightly than oligos containing guanine or thymine ( [13]  ; Bryan Wang and COP, unpublished data).	transcription
60017	3	335556	7	NULL	NULL	0	NULL	Zif268	Chemical		bind					guanine oligos	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_structure_4_10_1171_s_103	8939742	Competition experiments and  Kd determinations also show that Zif268 binds oligos with adenine or cytosine at these positions about 5 to 10-fold more tightly than oligos containing guanine or thymine ( [13]  ; Bryan Wang and COP, unpublished data).	transcription
60018	4	335556	7	NULL	NULL	0	NULL	Zif268	Chemical		bind					thymine oligos	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_structure_4_10_1171_s_103	8939742	Competition experiments and  Kd determinations also show that Zif268 binds oligos with adenine or cytosine at these positions about 5 to 10-fold more tightly than oligos containing guanine or thymine ( [13]  ; Bryan Wang and COP, unpublished data).	transcription
60019	5	335556	7	NULL	NULL	0	NULL	statement 1	Process	binding of	is stronger than					statement 3	Process	binding of			NULL		0	NULL	NULL	NULL	gw60_structure_4_10_1171_s_103	8939742	Competition experiments and  Kd determinations also show that Zif268 binds oligos with adenine or cytosine at these positions about 5 to 10-fold more tightly than oligos containing guanine or thymine ( [13]  ; Bryan Wang and COP, unpublished data).	transcription
60020	6	335556	7	NULL	NULL	0	NULL	statement 1	Process	binding of	is stronger than					statement 4	Process	binding of			NULL		0	NULL	NULL	NULL	gw60_structure_4_10_1171_s_103	8939742	Competition experiments and  Kd determinations also show that Zif268 binds oligos with adenine or cytosine at these positions about 5 to 10-fold more tightly than oligos containing guanine or thymine ( [13]  ; Bryan Wang and COP, unpublished data).	transcription
60021	7	335556	7	NULL	NULL	0	NULL	statement 2	Process	binding of	is stronger than					statement 3	Process	binding of			NULL		0	NULL	NULL	NULL	gw60_structure_4_10_1171_s_103	8939742	Competition experiments and  Kd determinations also show that Zif268 binds oligos with adenine or cytosine at these positions about 5 to 10-fold more tightly than oligos containing guanine or thymine ( [13]  ; Bryan Wang and COP, unpublished data).	transcription
60022	8	335556	7	NULL	NULL	0	NULL	statement 2	Process	binding of	is stronger than					statement 4	Process	binding of			NULL		0	NULL	NULL	NULL	gw60_structure_4_10_1171_s_103	8939742	Competition experiments and  Kd determinations also show that Zif268 binds oligos with adenine or cytosine at these positions about 5 to 10-fold more tightly than oligos containing guanine or thymine ( [13]  ; Bryan Wang and COP, unpublished data).	transcription
55105	1	335557	5	NULL	NULL	0	NULL	cytochrome c		released	work together with					Apaf-1					NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_173	9689121	The released cytochrome  c could work together with Apaf-1, caspase-9, and increasing concentrations of adenine deoxynuclesoside 5''-triphosphates to start a feed forward amplification cascade of caspase activation.	transcription
55106	2	335557	5	NULL	NULL	0	NULL	cytochrome c		released	work together with					caspase-9					NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_173	9689121	The released cytochrome  c could work together with Apaf-1, caspase-9, and increasing concentrations of adenine deoxynuclesoside 5''-triphosphates to start a feed forward amplification cascade of caspase activation.	transcription
55107	3	335557	5	NULL	NULL	0	NULL	cytochrome c		released	work together with					adenine deoxynuclesoside 5''-triphosphates		increasing concentrations of			NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_173	9689121	The released cytochrome  c could work together with Apaf-1, caspase-9, and increasing concentrations of adenine deoxynuclesoside 5''-triphosphates to start a feed forward amplification cascade of caspase activation.	transcription
55108	4	335557	5	NULL	NULL	0	NULL	statement 1			occurs along with					statement 2					NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_173	9689121	The released cytochrome  c could work together with Apaf-1, caspase-9, and increasing concentrations of adenine deoxynuclesoside 5''-triphosphates to start a feed forward amplification cascade of caspase activation.	transcription
55109	5	335557	5	NULL	NULL	0	NULL	statement 2			occurs along with					statement 3					NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_173	9689121	The released cytochrome  c could work together with Apaf-1, caspase-9, and increasing concentrations of adenine deoxynuclesoside 5''-triphosphates to start a feed forward amplification cascade of caspase activation.	transcription
55110	6	335557	5	NULL	NULL	0	NULL	statement 4			starts					caspase		feed forward amplification cascade of;;activation of			NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_173	9689121	The released cytochrome  c could work together with Apaf-1, caspase-9, and increasing concentrations of adenine deoxynuclesoside 5''-triphosphates to start a feed forward amplification cascade of caspase activation.	transcription
55111	7	335557	5	NULL	NULL	0	NULL	statement 5			starts					caspase		feed forward amplification cascade of;;activation of			NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_173	9689121	The released cytochrome  c could work together with Apaf-1, caspase-9, and increasing concentrations of adenine deoxynuclesoside 5''-triphosphates to start a feed forward amplification cascade of caspase activation.	transcription
60023	1	335557	7	NULL	NULL	0	NULL	cytochrome c	GP		start					caspase activation	Process	feed forward amplification cascade of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_173	9689121	The released cytochrome  c could work together with Apaf-1, caspase-9, and increasing concentrations of adenine deoxynuclesoside 5''-triphosphates to start a feed forward amplification cascade of caspase activation.	transcription
60024	2	335557	7	NULL	NULL	0	NULL	statement 1	Process		work along with					Apaf-1	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_173	9689121	The released cytochrome  c could work together with Apaf-1, caspase-9, and increasing concentrations of adenine deoxynuclesoside 5''-triphosphates to start a feed forward amplification cascade of caspase activation.	transcription
60025	3	335557	7	NULL	NULL	0	NULL	statement 1	Process		work along with					caspase-9	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_173	9689121	The released cytochrome  c could work together with Apaf-1, caspase-9, and increasing concentrations of adenine deoxynuclesoside 5''-triphosphates to start a feed forward amplification cascade of caspase activation.	transcription
60026	4	335557	7	NULL	NULL	0	NULL	statement 1	Process		work along with					adenine deoxynuclesoside 5''-triphosphates	Chemical				NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_173	9689121	The released cytochrome  c could work together with Apaf-1, caspase-9, and increasing concentrations of adenine deoxynuclesoside 5''-triphosphates to start a feed forward amplification cascade of caspase activation.	transcription
55112	1	335558	5	NULL	NULL	0	NULL	Apaf-1			bind					caspase-9					NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_178	9689121	However, the binding of Apaf-1 to caspase-9, and caspase-3, in the presence of high concentrations of adenine deoxynucleoside 5''-triphosphates and small amounts of released cytochrome  c, leads to the cleavage of caspase-3, converting it to an active autocatalytic protease, in a process analogous to blood clotting.	transcription
55113	2	335558	5	NULL	NULL	0	NULL	Apaf-1			bind					caspase-3					NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_178	9689121	However, the binding of Apaf-1 to caspase-9, and caspase-3, in the presence of high concentrations of adenine deoxynucleoside 5''-triphosphates and small amounts of released cytochrome  c, leads to the cleavage of caspase-3, converting it to an active autocatalytic protease, in a process analogous to blood clotting.	transcription
55114	3	335558	5	NULL	NULL	0	NULL	statement 1			in the presence of					adenine deoxynucleoside 5''-triphosphates		high concentrations of			NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_178	9689121	However, the binding of Apaf-1 to caspase-9, and caspase-3, in the presence of high concentrations of adenine deoxynucleoside 5''-triphosphates and small amounts of released cytochrome  c, leads to the cleavage of caspase-3, converting it to an active autocatalytic protease, in a process analogous to blood clotting.	transcription
55115	4	335558	5	NULL	NULL	0	NULL	statement 2			in the presence of					adenine deoxynucleoside 5''-triphosphates		high concentrations of			NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_178	9689121	However, the binding of Apaf-1 to caspase-9, and caspase-3, in the presence of high concentrations of adenine deoxynucleoside 5''-triphosphates and small amounts of released cytochrome  c, leads to the cleavage of caspase-3, converting it to an active autocatalytic protease, in a process analogous to blood clotting.	transcription
55116	5	335558	5	NULL	NULL	0	NULL	statement 1			in the presence of					cytochrome c		small amounts of;;released			NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_178	9689121	However, the binding of Apaf-1 to caspase-9, and caspase-3, in the presence of high concentrations of adenine deoxynucleoside 5''-triphosphates and small amounts of released cytochrome  c, leads to the cleavage of caspase-3, converting it to an active autocatalytic protease, in a process analogous to blood clotting.	transcription
55117	6	335558	5	NULL	NULL	0	NULL	statement 2			in the presence of					cytochrome c		small amounts of;;released			NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_178	9689121	However, the binding of Apaf-1 to caspase-9, and caspase-3, in the presence of high concentrations of adenine deoxynucleoside 5''-triphosphates and small amounts of released cytochrome  c, leads to the cleavage of caspase-3, converting it to an active autocatalytic protease, in a process analogous to blood clotting.	transcription
55118	7	335558	5	NULL	NULL	0	NULL	caspase-3			undergoes					cleavage					NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_178	9689121	However, the binding of Apaf-1 to caspase-9, and caspase-3, in the presence of high concentrations of adenine deoxynucleoside 5''-triphosphates and small amounts of released cytochrome  c, leads to the cleavage of caspase-3, converting it to an active autocatalytic protease, in a process analogous to blood clotting.	transcription
55119	8	335558	5	NULL	NULL	0	NULL	statement 7			is converted to					protease		active;;autocatalytic			NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_178	9689121	However, the binding of Apaf-1 to caspase-9, and caspase-3, in the presence of high concentrations of adenine deoxynucleoside 5''-triphosphates and small amounts of released cytochrome  c, leads to the cleavage of caspase-3, converting it to an active autocatalytic protease, in a process analogous to blood clotting.	transcription
55120	9	335558	5	NULL	NULL	0	NULL	statement 8			is analogous to					blood		clotting of			NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_178	9689121	However, the binding of Apaf-1 to caspase-9, and caspase-3, in the presence of high concentrations of adenine deoxynucleoside 5''-triphosphates and small amounts of released cytochrome  c, leads to the cleavage of caspase-3, converting it to an active autocatalytic protease, in a process analogous to blood clotting.	transcription
55121	10	335558	5	NULL	NULL	0	NULL	statement 3			leads to					statement 7					NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_178	9689121	However, the binding of Apaf-1 to caspase-9, and caspase-3, in the presence of high concentrations of adenine deoxynucleoside 5''-triphosphates and small amounts of released cytochrome  c, leads to the cleavage of caspase-3, converting it to an active autocatalytic protease, in a process analogous to blood clotting.	transcription
55122	11	335558	5	NULL	NULL	0	NULL	statement 4			leads to					statement 7					NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_178	9689121	However, the binding of Apaf-1 to caspase-9, and caspase-3, in the presence of high concentrations of adenine deoxynucleoside 5''-triphosphates and small amounts of released cytochrome  c, leads to the cleavage of caspase-3, converting it to an active autocatalytic protease, in a process analogous to blood clotting.	transcription
55123	12	335558	5	NULL	NULL	0	NULL	statement 5			leads to					statement 7					NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_178	9689121	However, the binding of Apaf-1 to caspase-9, and caspase-3, in the presence of high concentrations of adenine deoxynucleoside 5''-triphosphates and small amounts of released cytochrome  c, leads to the cleavage of caspase-3, converting it to an active autocatalytic protease, in a process analogous to blood clotting.	transcription
55124	13	335558	5	NULL	NULL	0	NULL	statement 6			leads to					statement 7					NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_178	9689121	However, the binding of Apaf-1 to caspase-9, and caspase-3, in the presence of high concentrations of adenine deoxynucleoside 5''-triphosphates and small amounts of released cytochrome  c, leads to the cleavage of caspase-3, converting it to an active autocatalytic protease, in a process analogous to blood clotting.	transcription
60027	1	335558	7	NULL	NULL	0	NULL	Apaf-1	GP		bind					caspase-9	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_178	9689121	However, the binding of Apaf-1 to caspase-9, and caspase-3, in the presence of high concentrations of adenine deoxynucleoside 5''-triphosphates and small amounts of released cytochrome  c, leads to the cleavage of caspase-3, converting it to an active autocatalytic protease, in a process analogous to blood clotting.	transcription
60028	2	335558	7	NULL	NULL	0	NULL	 Apaf-1	GP		bind					caspase-3	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_178	9689121	However, the binding of Apaf-1 to caspase-9, and caspase-3, in the presence of high concentrations of adenine deoxynucleoside 5''-triphosphates and small amounts of released cytochrome  c, leads to the cleavage of caspase-3, converting it to an active autocatalytic protease, in a process analogous to blood clotting.	transcription
60029	3	335558	7	NULL	NULL	0	NULL	statement 1	Process		in the presence of					adenine deoxynucleoside 5''-triphosphates	Chemical				NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_178	9689121	However, the binding of Apaf-1 to caspase-9, and caspase-3, in the presence of high concentrations of adenine deoxynucleoside 5''-triphosphates and small amounts of released cytochrome  c, leads to the cleavage of caspase-3, converting it to an active autocatalytic protease, in a process analogous to blood clotting.	transcription
60030	4	335558	7	NULL	NULL	0	NULL	statement 2	Process		in the presence of					adenine deoxynucleoside 5''-triphosphates	Chemical				NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_178	9689121	However, the binding of Apaf-1 to caspase-9, and caspase-3, in the presence of high concentrations of adenine deoxynucleoside 5''-triphosphates and small amounts of released cytochrome  c, leads to the cleavage of caspase-3, converting it to an active autocatalytic protease, in a process analogous to blood clotting.	transcription
60031	5	335558	7	NULL	NULL	0	NULL	 cytochrome c	GP		leads to					caspase-3	GP	cleavage of			NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_178	9689121	However, the binding of Apaf-1 to caspase-9, and caspase-3, in the presence of high concentrations of adenine deoxynucleoside 5''-triphosphates and small amounts of released cytochrome  c, leads to the cleavage of caspase-3, converting it to an active autocatalytic protease, in a process analogous to blood clotting.	transcription
60032	6	335558	7	NULL	NULL	0	NULL	statement 5	Process		converts it to					autocatalytic protease	GP	active			NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_178	9689121	However, the binding of Apaf-1 to caspase-9, and caspase-3, in the presence of high concentrations of adenine deoxynucleoside 5''-triphosphates and small amounts of released cytochrome  c, leads to the cleavage of caspase-3, converting it to an active autocatalytic protease, in a process analogous to blood clotting.	transcription
60033	7	335558	7	NULL	NULL	0	NULL	statement 6	Process		is analogous to					blood clotting	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_16_9567_s_178	9689121	However, the binding of Apaf-1 to caspase-9, and caspase-3, in the presence of high concentrations of adenine deoxynucleoside 5''-triphosphates and small amounts of released cytochrome  c, leads to the cleavage of caspase-3, converting it to an active autocatalytic protease, in a process analogous to blood clotting.	transcription
60034	1	335559	7	NULL	NULL	0	NULL	adenine 7	Chemical		modified to					purine	Chemical				NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9244_s_179	9689065	Modification of adenine  7 to a purine or hypoxanthine only slightly affects protein binding ( 2), and even the Tyr85His protein binds with similar affinity, provided that the histidine ring is protonated to make the hydrogen bond with phosphate  5 ( 18).	transcription
60035	2	335559	7	NULL	NULL	0	NULL	adenine 7 	Chemical		modified to					hypoxanthine	Chemical				NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9244_s_179	9689065	Modification of adenine  7 to a purine or hypoxanthine only slightly affects protein binding ( 2), and even the Tyr85His protein binds with similar affinity, provided that the histidine ring is protonated to make the hydrogen bond with phosphate  5 ( 18).	transcription
60036	3	335559	7	NULL	NULL	0	NULL	statement 1	Process		affects		slightly			protein	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_16_9244_s_179	9689065	Modification of adenine  7 to a purine or hypoxanthine only slightly affects protein binding ( 2), and even the Tyr85His protein binds with similar affinity, provided that the histidine ring is protonated to make the hydrogen bond with phosphate  5 ( 18).	transcription
60037	4	335559	7	NULL	NULL	0	NULL	statement 2	Process		affects		slightly			protein	GP	binding of			NULL		0	NULL	NULL	NULL	gw60_pnas_95_16_9244_s_179	9689065	Modification of adenine  7 to a purine or hypoxanthine only slightly affects protein binding ( 2), and even the Tyr85His protein binds with similar affinity, provided that the histidine ring is protonated to make the hydrogen bond with phosphate  5 ( 18).	transcription
55127	1	335560	5	NULL	NULL	0	NULL	TSA			is an inhibitor of					HDAC					NULL		0	NULL	NULL	NULL	gw60_pnas_97_25_13708_s_25	11095743	Of these, Rpd3p and Hda1p are sensitive to the HDAC inhibitor TSA. Hos3p and Sir2p are TSA-insensitive, Sir2p is activated by nicotinamide adenine dinucleotide (NAD), and little is known about Hos1p and Hos2p ( 5,  6).	transcription
55128	2	335560	5	NULL	NULL	0	NULL	Rpd3p			is sensitive to					TSA					NULL		0	NULL	NULL	NULL	gw60_pnas_97_25_13708_s_25	11095743	Of these, Rpd3p and Hda1p are sensitive to the HDAC inhibitor TSA. Hos3p and Sir2p are TSA-insensitive, Sir2p is activated by nicotinamide adenine dinucleotide (NAD), and little is known about Hos1p and Hos2p ( 5,  6).	transcription
55129	3	335560	5	NULL	NULL	0	NULL	Hda1p			is sensitive to					TSA					NULL		0	NULL	NULL	NULL	gw60_pnas_97_25_13708_s_25	11095743	Of these, Rpd3p and Hda1p are sensitive to the HDAC inhibitor TSA. Hos3p and Sir2p are TSA-insensitive, Sir2p is activated by nicotinamide adenine dinucleotide (NAD), and little is known about Hos1p and Hos2p ( 5,  6).	transcription
55130	4	335560	5	NULL	NULL	0	NULL	Hos3p			is insensitive to					TSA					NULL		0	NULL	NULL	NULL	gw60_pnas_97_25_13708_s_25	11095743	Of these, Rpd3p and Hda1p are sensitive to the HDAC inhibitor TSA. Hos3p and Sir2p are TSA-insensitive, Sir2p is activated by nicotinamide adenine dinucleotide (NAD), and little is known about Hos1p and Hos2p ( 5,  6).	transcription
55131	5	335560	5	NULL	NULL	0	NULL	Sir2p			is insensitive to					TSA					NULL		0	NULL	NULL	NULL	gw60_pnas_97_25_13708_s_25	11095743	Of these, Rpd3p and Hda1p are sensitive to the HDAC inhibitor TSA. Hos3p and Sir2p are TSA-insensitive, Sir2p is activated by nicotinamide adenine dinucleotide (NAD), and little is known about Hos1p and Hos2p ( 5,  6).	transcription
55132	6	335560	5	NULL	NULL	0	NULL	Sir2p			is activated by					NAD					NULL		0	NULL	NULL	NULL	gw60_pnas_97_25_13708_s_25	11095743	Of these, Rpd3p and Hda1p are sensitive to the HDAC inhibitor TSA. Hos3p and Sir2p are TSA-insensitive, Sir2p is activated by nicotinamide adenine dinucleotide (NAD), and little is known about Hos1p and Hos2p ( 5,  6).	transcription
55133	7	335560	5	NULL	NULL	0	NULL	NAD			is					nicotinamide adenine dinucleotide					NULL		0	NULL	NULL	NULL	gw60_pnas_97_25_13708_s_25	11095743	Of these, Rpd3p and Hda1p are sensitive to the HDAC inhibitor TSA. Hos3p and Sir2p are TSA-insensitive, Sir2p is activated by nicotinamide adenine dinucleotide (NAD), and little is known about Hos1p and Hos2p ( 5,  6).	transcription
60038	1	335560	7	NULL	NULL	0	NULL	Rpd3p	GP		is sensitive to					TSA	Chemical				NULL		0	NULL	NULL	NULL	gw60_pnas_97_25_13708_s_25	11095743	Of these, Rpd3p and Hda1p are sensitive to the HDAC inhibitor TSA. Hos3p and Sir2p are TSA-insensitive, Sir2p is activated by nicotinamide adenine dinucleotide (NAD), and little is known about Hos1p and Hos2p ( 5,  6).	transcription
60039	2	335560	7	NULL	NULL	0	NULL	Hda1p	GP		is sensitive to					TSA	Chemical				NULL		0	NULL	NULL	NULL	gw60_pnas_97_25_13708_s_25	11095743	Of these, Rpd3p and Hda1p are sensitive to the HDAC inhibitor TSA. Hos3p and Sir2p are TSA-insensitive, Sir2p is activated by nicotinamide adenine dinucleotide (NAD), and little is known about Hos1p and Hos2p ( 5,  6).	transcription
60040	3	335560	7	NULL	NULL	0	NULL	TSA	Chemical		is a type of					HDAC inhibitor	Chemical				NULL		0	NULL	NULL	NULL	gw60_pnas_97_25_13708_s_25	11095743	Of these, Rpd3p and Hda1p are sensitive to the HDAC inhibitor TSA. Hos3p and Sir2p are TSA-insensitive, Sir2p is activated by nicotinamide adenine dinucleotide (NAD), and little is known about Hos1p and Hos2p ( 5,  6).	transcription
60041	4	335560	7	NULL	NULL	0	NULL	Hos3p	GP		is insensitive to					TSA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_25_13708_s_25	11095743	Of these, Rpd3p and Hda1p are sensitive to the HDAC inhibitor TSA. Hos3p and Sir2p are TSA-insensitive, Sir2p is activated by nicotinamide adenine dinucleotide (NAD), and little is known about Hos1p and Hos2p ( 5,  6).	transcription
60042	5	335560	7	NULL	NULL	0	NULL	Sir2p	GP		is insensitive to					TSA	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_25_13708_s_25	11095743	Of these, Rpd3p and Hda1p are sensitive to the HDAC inhibitor TSA. Hos3p and Sir2p are TSA-insensitive, Sir2p is activated by nicotinamide adenine dinucleotide (NAD), and little is known about Hos1p and Hos2p ( 5,  6).	transcription
60043	6	335560	7	NULL	NULL	0	NULL	NAD	Chemical		activates					Sir2p	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_97_25_13708_s_25	11095743	Of these, Rpd3p and Hda1p are sensitive to the HDAC inhibitor TSA. Hos3p and Sir2p are TSA-insensitive, Sir2p is activated by nicotinamide adenine dinucleotide (NAD), and little is known about Hos1p and Hos2p ( 5,  6).	transcription
60044	7	335560	7	NULL	NULL	0	NULL	NAD	Chemical		is					nicotinamide adenine dinucleotide	Chemical				NULL		0	NULL	NULL	NULL	gw60_pnas_97_25_13708_s_25	11095743	Of these, Rpd3p and Hda1p are sensitive to the HDAC inhibitor TSA. Hos3p and Sir2p are TSA-insensitive, Sir2p is activated by nicotinamide adenine dinucleotide (NAD), and little is known about Hos1p and Hos2p ( 5,  6).	transcription
55134	1	335561	5	NULL	NULL	0	NULL	guanosine			incorporated into					nucleic acids					NULL		0	NULL	NULL	NULL	gw60_pnas_98_8_4593_s_171	11287638	Imm-H suppressed only the incorporation of guanosine into nucleic acids (Fig.  5) with no effect on adenine and guanine phosphoribosyltransferases, dCK, adenosine kinase, or the enzymes of RNA and DNA synthesis, consistent with selective inhibition of PNP.	transcription
55135	2	335561	5	NULL	NULL	0	NULL	Imm-H			suppress					statement 1					NULL		0	NULL	NULL	NULL	gw60_pnas_98_8_4593_s_171	11287638	Imm-H suppressed only the incorporation of guanosine into nucleic acids (Fig.  5) with no effect on adenine and guanine phosphoribosyltransferases, dCK, adenosine kinase, or the enzymes of RNA and DNA synthesis, consistent with selective inhibition of PNP.	transcription
55140	3	335561	5	NULL	NULL	0	NULL	statement 2			does not effect					adenine phosphoribosyltransferases					NULL		0	NULL	NULL	NULL	gw60_pnas_98_8_4593_s_171	11287638	Imm-H suppressed only the incorporation of guanosine into nucleic acids (Fig.  5) with no effect on adenine and guanine phosphoribosyltransferases, dCK, adenosine kinase, or the enzymes of RNA and DNA synthesis, consistent with selective inhibition of PNP.	transcription
55141	4	335561	5	NULL	NULL	0	NULL	statement 2			does not effect					guanine phosphoribosyltransferases					NULL		0	NULL	NULL	NULL	gw60_pnas_98_8_4593_s_171	11287638	Imm-H suppressed only the incorporation of guanosine into nucleic acids (Fig.  5) with no effect on adenine and guanine phosphoribosyltransferases, dCK, adenosine kinase, or the enzymes of RNA and DNA synthesis, consistent with selective inhibition of PNP.	transcription
55142	5	335561	5	NULL	NULL	0	NULL	statement 2			does not effect					dCK					NULL		0	NULL	NULL	NULL	gw60_pnas_98_8_4593_s_171	11287638	Imm-H suppressed only the incorporation of guanosine into nucleic acids (Fig.  5) with no effect on adenine and guanine phosphoribosyltransferases, dCK, adenosine kinase, or the enzymes of RNA and DNA synthesis, consistent with selective inhibition of PNP.	transcription
55143	6	335561	5	NULL	NULL	0	NULL	statement 2			does not effect					adenosine kinase					NULL		0	NULL	NULL	NULL	gw60_pnas_98_8_4593_s_171	11287638	Imm-H suppressed only the incorporation of guanosine into nucleic acids (Fig.  5) with no effect on adenine and guanine phosphoribosyltransferases, dCK, adenosine kinase, or the enzymes of RNA and DNA synthesis, consistent with selective inhibition of PNP.	transcription
55144	7	335561	5	NULL	NULL	0	NULL	statement 2			does not effect					enzymes of RNA synthesis					NULL		0	NULL	NULL	NULL	gw60_pnas_98_8_4593_s_171	11287638	Imm-H suppressed only the incorporation of guanosine into nucleic acids (Fig.  5) with no effect on adenine and guanine phosphoribosyltransferases, dCK, adenosine kinase, or the enzymes of RNA and DNA synthesis, consistent with selective inhibition of PNP.	transcription
55145	8	335561	5	NULL	NULL	0	NULL	statement 2			does not effect					enzymes of DNA synthesis					NULL		0	NULL	NULL	NULL	gw60_pnas_98_8_4593_s_171	11287638	Imm-H suppressed only the incorporation of guanosine into nucleic acids (Fig.  5) with no effect on adenine and guanine phosphoribosyltransferases, dCK, adenosine kinase, or the enzymes of RNA and DNA synthesis, consistent with selective inhibition of PNP.	transcription
55146	9	335561	5	NULL	NULL	0	NULL	statement 2			inhibits		selectively			PNP					NULL		0	NULL	NULL	NULL	gw60_pnas_98_8_4593_s_171	11287638	Imm-H suppressed only the incorporation of guanosine into nucleic acids (Fig.  5) with no effect on adenine and guanine phosphoribosyltransferases, dCK, adenosine kinase, or the enzymes of RNA and DNA synthesis, consistent with selective inhibition of PNP.	transcription
60078	1	335561	7	NULL	NULL	0	NULL	guanosine	NucleicAcid		incorporated into					nucleic acids	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_pnas_98_8_4593_s_171	11287638	Imm-H suppressed only the incorporation of guanosine into nucleic acids (Fig.  5) with no effect on adenine and guanine phosphoribosyltransferases, dCK, adenosine kinase, or the enzymes of RNA and DNA synthesis, consistent with selective inhibition of PNP.	transcription
60079	2	335561	7	NULL	NULL	0	NULL	Imm-H	Chemical		suppress					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_98_8_4593_s_171	11287638	Imm-H suppressed only the incorporation of guanosine into nucleic acids (Fig.  5) with no effect on adenine and guanine phosphoribosyltransferases, dCK, adenosine kinase, or the enzymes of RNA and DNA synthesis, consistent with selective inhibition of PNP.	transcription
60080	3	335561	7	NULL	NULL	0	NULL	statement 2	Process		does not effect					adenine  phosphoribosyltransferase	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_98_8_4593_s_171	11287638	Imm-H suppressed only the incorporation of guanosine into nucleic acids (Fig.  5) with no effect on adenine and guanine phosphoribosyltransferases, dCK, adenosine kinase, or the enzymes of RNA and DNA synthesis, consistent with selective inhibition of PNP.	transcription
60081	4	335561	7	NULL	NULL	0	NULL	statement 2	Process		does not effect					guanine phosphoribosyltransferase	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_98_8_4593_s_171	11287638	Imm-H suppressed only the incorporation of guanosine into nucleic acids (Fig.  5) with no effect on adenine and guanine phosphoribosyltransferases, dCK, adenosine kinase, or the enzymes of RNA and DNA synthesis, consistent with selective inhibition of PNP.	transcription
60082	5	335561	7	NULL	NULL	0	NULL	statement 2	Process		does not effect					dCK	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_98_8_4593_s_171	11287638	Imm-H suppressed only the incorporation of guanosine into nucleic acids (Fig.  5) with no effect on adenine and guanine phosphoribosyltransferases, dCK, adenosine kinase, or the enzymes of RNA and DNA synthesis, consistent with selective inhibition of PNP.	transcription
60083	6	335561	7	NULL	NULL	0	NULL	statement 2	Process		does not effect					adenosine kinase	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_98_8_4593_s_171	11287638	Imm-H suppressed only the incorporation of guanosine into nucleic acids (Fig.  5) with no effect on adenine and guanine phosphoribosyltransferases, dCK, adenosine kinase, or the enzymes of RNA and DNA synthesis, consistent with selective inhibition of PNP.	transcription
55147	1	335562	5	NULL	NULL	0	NULL	CtrA			controls		directly			ccrM gene		expression of			NULL	late in the cell cycle	NULL	NULL	NULL	NULL	gw60_pnas_99_7_4632_s_205	11930012	Consistent with previous results ( 5,  8), we found that CtrA directly controls expression of the essential gene  ccrM, encoding an adenine DNA methyltransferase, late in the cell cycle.	transcription
55148	2	335562	5	NULL	NULL	0	NULL	ccrM gene			encodes					adenine DNA methyltransferase					NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_7_4632_s_205	11930012	Consistent with previous results ( 5,  8), we found that CtrA directly controls expression of the essential gene  ccrM, encoding an adenine DNA methyltransferase, late in the cell cycle.	transcription
60084	1	335562	7	NULL	NULL	0	NULL	CtrA	GP		controls expression of		directly			ccrM gene	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_99_7_4632_s_205	11930012	Consistent with previous results ( 5,  8), we found that CtrA directly controls expression of the essential gene  ccrM, encoding an adenine DNA methyltransferase, late in the cell cycle.	transcription
60085	2	335562	7	NULL	NULL	0	NULL	ccrM gene	GP		encode					adenine DNA methyltransferase	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_99_7_4632_s_205	11930012	Consistent with previous results ( 5,  8), we found that CtrA directly controls expression of the essential gene  ccrM, encoding an adenine DNA methyltransferase, late in the cell cycle.	transcription
60086	3	335562	7	NULL	NULL	0	NULL	statement 2	Process		occur during					late cell cycle	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_99_7_4632_s_205	11930012	Consistent with previous results ( 5,  8), we found that CtrA directly controls expression of the essential gene  ccrM, encoding an adenine DNA methyltransferase, late in the cell cycle.	transcription
55154	1	335563	5	NULL	NULL	0	NULL	erythro-9-(2-hydroxy-3-nonyl-)-adenine			block					adenosine deaminase					NULL		0	NULL	NULL	NULL	abs-batch0580-0599_j-physiol_570_pt-2_16284071_s_9	16284071	Blockade of adenosine deaminase (with erythro-9-(2-hydroxy-3-nonyl-)-adenine,  5 microM), adenosine kinase (with iodotubericidine, 10 microM) and adenosine  transport (with n-nitrobenzylthioinosine, 1 microM) increased interstitial  adenosine but the increase was unrelated to hypoxia or diameter.	transcription
55155	2	335563	5	NULL	NULL	0	NULL	statement 1			increases					adenosine		interstitial			NULL		0	NULL	NULL	NULL	abs-batch0580-0599_j-physiol_570_pt-2_16284071_s_9	16284071	Blockade of adenosine deaminase (with erythro-9-(2-hydroxy-3-nonyl-)-adenine,  5 microM), adenosine kinase (with iodotubericidine, 10 microM) and adenosine  transport (with n-nitrobenzylthioinosine, 1 microM) increased interstitial  adenosine but the increase was unrelated to hypoxia or diameter.	transcription
55156	3	335563	5	NULL	NULL	0	NULL	statement 2			unrelated to					hypoxia					NULL		0	NULL	NULL	NULL	abs-batch0580-0599_j-physiol_570_pt-2_16284071_s_9	16284071	Blockade of adenosine deaminase (with erythro-9-(2-hydroxy-3-nonyl-)-adenine,  5 microM), adenosine kinase (with iodotubericidine, 10 microM) and adenosine  transport (with n-nitrobenzylthioinosine, 1 microM) increased interstitial  adenosine but the increase was unrelated to hypoxia or diameter.	transcription
55157	4	335563	5	NULL	NULL	0	NULL	statement 2			unrelated to					diameter					NULL		0	NULL	NULL	NULL	abs-batch0580-0599_j-physiol_570_pt-2_16284071_s_9	16284071	Blockade of adenosine deaminase (with erythro-9-(2-hydroxy-3-nonyl-)-adenine,  5 microM), adenosine kinase (with iodotubericidine, 10 microM) and adenosine  transport (with n-nitrobenzylthioinosine, 1 microM) increased interstitial  adenosine but the increase was unrelated to hypoxia or diameter.	transcription
55158	5	335563	5	NULL	NULL	0	NULL	statement 3			is an alternative to					statement 4					NULL		0	NULL	NULL	NULL	abs-batch0580-0599_j-physiol_570_pt-2_16284071_s_9	16284071	Blockade of adenosine deaminase (with erythro-9-(2-hydroxy-3-nonyl-)-adenine,  5 microM), adenosine kinase (with iodotubericidine, 10 microM) and adenosine  transport (with n-nitrobenzylthioinosine, 1 microM) increased interstitial  adenosine but the increase was unrelated to hypoxia or diameter.	transcription
55159	6	335563	5	NULL	NULL	0	NULL	iodotubericidine			block					adenosine kinase					NULL		0	NULL	NULL	NULL	abs-batch0580-0599_j-physiol_570_pt-2_16284071_s_9	16284071	Blockade of adenosine deaminase (with erythro-9-(2-hydroxy-3-nonyl-)-adenine,  5 microM), adenosine kinase (with iodotubericidine, 10 microM) and adenosine  transport (with n-nitrobenzylthioinosine, 1 microM) increased interstitial  adenosine but the increase was unrelated to hypoxia or diameter.	transcription
55160	7	335563	5	NULL	NULL	0	NULL	statement 6			increases					adenosine		interstitial			NULL		0	NULL	NULL	NULL	abs-batch0580-0599_j-physiol_570_pt-2_16284071_s_9	16284071	Blockade of adenosine deaminase (with erythro-9-(2-hydroxy-3-nonyl-)-adenine,  5 microM), adenosine kinase (with iodotubericidine, 10 microM) and adenosine  transport (with n-nitrobenzylthioinosine, 1 microM) increased interstitial  adenosine but the increase was unrelated to hypoxia or diameter.	transcription
55161	8	335563	5	NULL	NULL	0	NULL	statement 7			unrelated to					hypoxia					NULL		0	NULL	NULL	NULL	abs-batch0580-0599_j-physiol_570_pt-2_16284071_s_9	16284071	Blockade of adenosine deaminase (with erythro-9-(2-hydroxy-3-nonyl-)-adenine,  5 microM), adenosine kinase (with iodotubericidine, 10 microM) and adenosine  transport (with n-nitrobenzylthioinosine, 1 microM) increased interstitial  adenosine but the increase was unrelated to hypoxia or diameter.	transcription
55162	9	335563	5	NULL	NULL	0	NULL	statement 7			unrelated to					diameter					NULL		0	NULL	NULL	NULL	abs-batch0580-0599_j-physiol_570_pt-2_16284071_s_9	16284071	Blockade of adenosine deaminase (with erythro-9-(2-hydroxy-3-nonyl-)-adenine,  5 microM), adenosine kinase (with iodotubericidine, 10 microM) and adenosine  transport (with n-nitrobenzylthioinosine, 1 microM) increased interstitial  adenosine but the increase was unrelated to hypoxia or diameter.	transcription
55163	10	335563	5	NULL	NULL	0	NULL	statement 8			is an alternative to					statement 9					NULL		0	NULL	NULL	NULL	abs-batch0580-0599_j-physiol_570_pt-2_16284071_s_9	16284071	Blockade of adenosine deaminase (with erythro-9-(2-hydroxy-3-nonyl-)-adenine,  5 microM), adenosine kinase (with iodotubericidine, 10 microM) and adenosine  transport (with n-nitrobenzylthioinosine, 1 microM) increased interstitial  adenosine but the increase was unrelated to hypoxia or diameter.	transcription
55164	11	335563	5	NULL	NULL	0	NULL	n-nitrobenzylthioinosine			block					adenosine transport					NULL		0	NULL	NULL	NULL	abs-batch0580-0599_j-physiol_570_pt-2_16284071_s_9	16284071	Blockade of adenosine deaminase (with erythro-9-(2-hydroxy-3-nonyl-)-adenine,  5 microM), adenosine kinase (with iodotubericidine, 10 microM) and adenosine  transport (with n-nitrobenzylthioinosine, 1 microM) increased interstitial  adenosine but the increase was unrelated to hypoxia or diameter.	transcription
55165	12	335563	5	NULL	NULL	0	NULL	statement 11			increases					adenosine		interstitial			NULL		0	NULL	NULL	NULL	abs-batch0580-0599_j-physiol_570_pt-2_16284071_s_9	16284071	Blockade of adenosine deaminase (with erythro-9-(2-hydroxy-3-nonyl-)-adenine,  5 microM), adenosine kinase (with iodotubericidine, 10 microM) and adenosine  transport (with n-nitrobenzylthioinosine, 1 microM) increased interstitial  adenosine but the increase was unrelated to hypoxia or diameter.	transcription
55166	13	335563	5	NULL	NULL	0	NULL	statement 12			unrelated to					hypoxia					NULL		0	NULL	NULL	NULL	abs-batch0580-0599_j-physiol_570_pt-2_16284071_s_9	16284071	Blockade of adenosine deaminase (with erythro-9-(2-hydroxy-3-nonyl-)-adenine,  5 microM), adenosine kinase (with iodotubericidine, 10 microM) and adenosine  transport (with n-nitrobenzylthioinosine, 1 microM) increased interstitial  adenosine but the increase was unrelated to hypoxia or diameter.	transcription
55167	14	335563	5	NULL	NULL	0	NULL	statement 12			unrelated to					diameter					NULL		0	NULL	NULL	NULL	abs-batch0580-0599_j-physiol_570_pt-2_16284071_s_9	16284071	Blockade of adenosine deaminase (with erythro-9-(2-hydroxy-3-nonyl-)-adenine,  5 microM), adenosine kinase (with iodotubericidine, 10 microM) and adenosine  transport (with n-nitrobenzylthioinosine, 1 microM) increased interstitial  adenosine but the increase was unrelated to hypoxia or diameter.	transcription
55168	15	335563	5	NULL	NULL	0	NULL	statement 13			is an alternative to					statement 14					NULL		0	NULL	NULL	NULL	abs-batch0580-0599_j-physiol_570_pt-2_16284071_s_9	16284071	Blockade of adenosine deaminase (with erythro-9-(2-hydroxy-3-nonyl-)-adenine,  5 microM), adenosine kinase (with iodotubericidine, 10 microM) and adenosine  transport (with n-nitrobenzylthioinosine, 1 microM) increased interstitial  adenosine but the increase was unrelated to hypoxia or diameter.	transcription
60087	1	335563	7	NULL	NULL	0	NULL	erythro-9-(2-hydroxy-3-nonyl-)-adenine	Chemical		blocks					adenosine deaminase	GP				NULL		0	NULL	NULL	NULL	abs-batch0580-0599_j-physiol_570_pt-2_16284071_s_9	16284071	Blockade of adenosine deaminase (with erythro-9-(2-hydroxy-3-nonyl-)-adenine,  5 microM), adenosine kinase (with iodotubericidine, 10 microM) and adenosine  transport (with n-nitrobenzylthioinosine, 1 microM) increased interstitial  adenosine but the increase was unrelated to hypoxia or diameter.	transcription
60088	2	335563	7	NULL	NULL	0	NULL	iodotubericidine	Chemical		blocks					adenosine kinase	GP				NULL		0	NULL	NULL	NULL	abs-batch0580-0599_j-physiol_570_pt-2_16284071_s_9	16284071	Blockade of adenosine deaminase (with erythro-9-(2-hydroxy-3-nonyl-)-adenine,  5 microM), adenosine kinase (with iodotubericidine, 10 microM) and adenosine  transport (with n-nitrobenzylthioinosine, 1 microM) increased interstitial  adenosine but the increase was unrelated to hypoxia or diameter.	transcription
60089	3	335563	7	NULL	NULL	0	NULL	 n-nitrobenzylthioinosine	Chemical		blocks					adenosine 	Process	transport of			NULL		0	NULL	NULL	NULL	abs-batch0580-0599_j-physiol_570_pt-2_16284071_s_9	16284071	Blockade of adenosine deaminase (with erythro-9-(2-hydroxy-3-nonyl-)-adenine,  5 microM), adenosine kinase (with iodotubericidine, 10 microM) and adenosine  transport (with n-nitrobenzylthioinosine, 1 microM) increased interstitial  adenosine but the increase was unrelated to hypoxia or diameter.	transcription
60090	4	335563	7	NULL	NULL	0	NULL	statement 1	Process		increase					 adenosine	NucleicAcid	interstitial			NULL		0	NULL	NULL	NULL	abs-batch0580-0599_j-physiol_570_pt-2_16284071_s_9	16284071	Blockade of adenosine deaminase (with erythro-9-(2-hydroxy-3-nonyl-)-adenine,  5 microM), adenosine kinase (with iodotubericidine, 10 microM) and adenosine  transport (with n-nitrobenzylthioinosine, 1 microM) increased interstitial  adenosine but the increase was unrelated to hypoxia or diameter.	transcription
60152	5	335563	7	NULL	NULL	0	NULL	statement 2	Process		increase					adenosine	NucleicAcid	interstitial			NULL		0	NULL	NULL	NULL	abs-batch0580-0599_j-physiol_570_pt-2_16284071_s_9	16284071	Blockade of adenosine deaminase (with erythro-9-(2-hydroxy-3-nonyl-)-adenine,  5 microM), adenosine kinase (with iodotubericidine, 10 microM) and adenosine  transport (with n-nitrobenzylthioinosine, 1 microM) increased interstitial  adenosine but the increase was unrelated to hypoxia or diameter.	transcription
60153	6	335563	7	NULL	NULL	0	NULL	statement 3	Process		increase					adenosine	NucleicAcid	interstitial			NULL		0	NULL	NULL	NULL	abs-batch0580-0599_j-physiol_570_pt-2_16284071_s_9	16284071	Blockade of adenosine deaminase (with erythro-9-(2-hydroxy-3-nonyl-)-adenine,  5 microM), adenosine kinase (with iodotubericidine, 10 microM) and adenosine  transport (with n-nitrobenzylthioinosine, 1 microM) increased interstitial  adenosine but the increase was unrelated to hypoxia or diameter.	transcription
60154	7	335563	7	NULL	NULL	0	NULL	statement 4	Process		is unrelated to					hypoxia	Process				NULL		0	NULL	NULL	NULL	abs-batch0580-0599_j-physiol_570_pt-2_16284071_s_9	16284071	Blockade of adenosine deaminase (with erythro-9-(2-hydroxy-3-nonyl-)-adenine,  5 microM), adenosine kinase (with iodotubericidine, 10 microM) and adenosine  transport (with n-nitrobenzylthioinosine, 1 microM) increased interstitial  adenosine but the increase was unrelated to hypoxia or diameter.	transcription
60155	8	335563	7	NULL	NULL	0	NULL	statement 5	Process		is unrelated to					hypoxia	Process				NULL		0	NULL	NULL	NULL	abs-batch0580-0599_j-physiol_570_pt-2_16284071_s_9	16284071	Blockade of adenosine deaminase (with erythro-9-(2-hydroxy-3-nonyl-)-adenine,  5 microM), adenosine kinase (with iodotubericidine, 10 microM) and adenosine  transport (with n-nitrobenzylthioinosine, 1 microM) increased interstitial  adenosine but the increase was unrelated to hypoxia or diameter.	transcription
60156	9	335563	7	NULL	NULL	0	NULL	statement 6	Process		is unrelated to					hypoxia	Process				NULL		0	NULL	NULL	NULL	abs-batch0580-0599_j-physiol_570_pt-2_16284071_s_9	16284071	Blockade of adenosine deaminase (with erythro-9-(2-hydroxy-3-nonyl-)-adenine,  5 microM), adenosine kinase (with iodotubericidine, 10 microM) and adenosine  transport (with n-nitrobenzylthioinosine, 1 microM) increased interstitial  adenosine but the increase was unrelated to hypoxia or diameter.	transcription
55220	1	335564	5	NULL	NULL	0	NULL	RNase L			undergoes		effectively			dimerization					NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biochem-(tokyo)_132_4_12359081_s_8	12359081	The results  suggest that 2-5A molecules modified at the 8-position of the third (from  the 5' terminus) adenine ring cause effective dimerization of RNase L  and thus increase the ability of RNase L activation.	transcription
55221	2	335564	5	NULL	NULL	0	NULL	2-5A molecules			is modified at								adenine ring		NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biochem-(tokyo)_132_4_12359081_s_8	12359081	The results  suggest that 2-5A molecules modified at the 8-position of the third (from  the 5' terminus) adenine ring cause effective dimerization of RNase L  and thus increase the ability of RNase L activation.	transcription
55222	3	335564	5	NULL	NULL	0	NULL	statement 2			results in					statement 1					NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biochem-(tokyo)_132_4_12359081_s_8	12359081	The results  suggest that 2-5A molecules modified at the 8-position of the third (from  the 5' terminus) adenine ring cause effective dimerization of RNase L  and thus increase the ability of RNase L activation.	transcription
55223	4	335564	5	NULL	NULL	0	NULL	statement 1			increases					RNase L		activation of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biochem-(tokyo)_132_4_12359081_s_8	12359081	The results  suggest that 2-5A molecules modified at the 8-position of the third (from  the 5' terminus) adenine ring cause effective dimerization of RNase L  and thus increase the ability of RNase L activation.	transcription
60157	1	335564	7	NULL	NULL	0	NULL				cause				2-5A molecules modified at the 8-position of the third adenine ring	RNase L	GP	effective dimerization of			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_j-biochem-(tokyo)_132_4_12359081_s_8	12359081	The results  suggest that 2-5A molecules modified at the 8-position of the third (from  the 5' terminus) adenine ring cause effective dimerization of RNase L  and thus increase the ability of RNase L activation.	transcription
60158	2	335564	7	NULL	NULL	0	NULL	statement 1	Process		increase					RNase L	GP	activation of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biochem-(tokyo)_132_4_12359081_s_8	12359081	The results  suggest that 2-5A molecules modified at the 8-position of the third (from  the 5' terminus) adenine ring cause effective dimerization of RNase L  and thus increase the ability of RNase L activation.	transcription
55224	1	335565	5	NULL	NULL	0	NULL	5 -AMP			bind					phosphorylase		liver			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_44_27569_s_200	8910343	The delta H b on 5 -AMP binding to liver phosphorylase  a is not so negative as when 5 -AMP binds to muscle isozyme ( 24), and the absence of some hydrogen bonds between the adenine N6 amino group of 5 -AMP and amino acids in the 315 to 325 loop might contribute to this.	transcription
55225	2	335565	5	NULL	NULL	0	NULL	5 -AMP			bind					isozyme		muscle			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_44_27569_s_200	8910343	The delta H b on 5 -AMP binding to liver phosphorylase  a is not so negative as when 5 -AMP binds to muscle isozyme ( 24), and the absence of some hydrogen bonds between the adenine N6 amino group of 5 -AMP and amino acids in the 315 to 325 loop might contribute to this.	transcription
60159	1	335565	7	NULL	NULL	0	NULL	5 -AMP	Chemical		bind					phosphorylase a	GP	liver			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_44_27569_s_200	8910343	The delta H b on 5 -AMP binding to liver phosphorylase  a is not so negative as when 5 -AMP binds to muscle isozyme ( 24), and the absence of some hydrogen bonds between the adenine N6 amino group of 5 -AMP and amino acids in the 315 to 325 loop might contribute to this.	transcription
60160	1	335566	7	NULL	NULL	0	NULL	G-protein	GP		is					heterotrimeric guanine nucleotide-binding protein	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_51_47785_s_341	11602596	The abbreviations used are:   G-protein, heterotrimeric guanine nucleotide-binding protein;  Gsalpha, the alpha subunit of G protein that stimulates adenylyl cyclase;  GTPgammaS, guanosine 5''-(gamma-thio) triphosphate;  THFA, 9-(tetrahydro-2-furyl) adenine;  CPA, 9-(cyclopentyl) adenine;  Ap(CH2)pp, alpha,beta-methylene adenosine 5''-triphosphate;  2''-d-3''-AMP, 2''-deoxyadenosine 3''-monophosphate;  3''-AMP, adenosine 3''-monophosphate.	transcription
60161	2	335566	7	NULL	NULL	0	NULL	Gsalpha	GP		is 					G protein	GP		alpha subunit of		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_51_47785_s_341	11602596	The abbreviations used are:   G-protein, heterotrimeric guanine nucleotide-binding protein;  Gsalpha, the alpha subunit of G protein that stimulates adenylyl cyclase;  GTPgammaS, guanosine 5''-(gamma-thio) triphosphate;  THFA, 9-(tetrahydro-2-furyl) adenine;  CPA, 9-(cyclopentyl) adenine;  Ap(CH2)pp, alpha,beta-methylene adenosine 5''-triphosphate;  2''-d-3''-AMP, 2''-deoxyadenosine 3''-monophosphate;  3''-AMP, adenosine 3''-monophosphate.	transcription
60162	3	335566	7	NULL	NULL	0	NULL	Gsalpha	GP		stimulates					adenylyl cyclase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_51_47785_s_341	11602596	The abbreviations used are:   G-protein, heterotrimeric guanine nucleotide-binding protein;  Gsalpha, the alpha subunit of G protein that stimulates adenylyl cyclase;  GTPgammaS, guanosine 5''-(gamma-thio) triphosphate;  THFA, 9-(tetrahydro-2-furyl) adenine;  CPA, 9-(cyclopentyl) adenine;  Ap(CH2)pp, alpha,beta-methylene adenosine 5''-triphosphate;  2''-d-3''-AMP, 2''-deoxyadenosine 3''-monophosphate;  3''-AMP, adenosine 3''-monophosphate.	transcription
60163	4	335566	7	NULL	NULL	0	NULL	GTPgammaS	GP		is					guanosine 5''-(gamma-thio) triphosphate	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_51_47785_s_341	11602596	The abbreviations used are:   G-protein, heterotrimeric guanine nucleotide-binding protein;  Gsalpha, the alpha subunit of G protein that stimulates adenylyl cyclase;  GTPgammaS, guanosine 5''-(gamma-thio) triphosphate;  THFA, 9-(tetrahydro-2-furyl) adenine;  CPA, 9-(cyclopentyl) adenine;  Ap(CH2)pp, alpha,beta-methylene adenosine 5''-triphosphate;  2''-d-3''-AMP, 2''-deoxyadenosine 3''-monophosphate;  3''-AMP, adenosine 3''-monophosphate.	transcription
60164	5	335566	7	NULL	NULL	0	NULL	THFA	Chemical		is					9-(tetrahydro-2-furyl) adenine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_51_47785_s_341	11602596	The abbreviations used are:   G-protein, heterotrimeric guanine nucleotide-binding protein;  Gsalpha, the alpha subunit of G protein that stimulates adenylyl cyclase;  GTPgammaS, guanosine 5''-(gamma-thio) triphosphate;  THFA, 9-(tetrahydro-2-furyl) adenine;  CPA, 9-(cyclopentyl) adenine;  Ap(CH2)pp, alpha,beta-methylene adenosine 5''-triphosphate;  2''-d-3''-AMP, 2''-deoxyadenosine 3''-monophosphate;  3''-AMP, adenosine 3''-monophosphate.	transcription
60165	6	335566	7	NULL	NULL	0	NULL	CPA	Chemical		is					9-(cyclopentyl) adenine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_51_47785_s_341	11602596	The abbreviations used are:   G-protein, heterotrimeric guanine nucleotide-binding protein;  Gsalpha, the alpha subunit of G protein that stimulates adenylyl cyclase;  GTPgammaS, guanosine 5''-(gamma-thio) triphosphate;  THFA, 9-(tetrahydro-2-furyl) adenine;  CPA, 9-(cyclopentyl) adenine;  Ap(CH2)pp, alpha,beta-methylene adenosine 5''-triphosphate;  2''-d-3''-AMP, 2''-deoxyadenosine 3''-monophosphate;  3''-AMP, adenosine 3''-monophosphate.	transcription
60166	7	335566	7	NULL	NULL	0	NULL	Ap(CH2)pp	Chemical		is					alpha,beta-methylene adenosine 5''-triphosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_51_47785_s_341	11602596	The abbreviations used are:   G-protein, heterotrimeric guanine nucleotide-binding protein;  Gsalpha, the alpha subunit of G protein that stimulates adenylyl cyclase;  GTPgammaS, guanosine 5''-(gamma-thio) triphosphate;  THFA, 9-(tetrahydro-2-furyl) adenine;  CPA, 9-(cyclopentyl) adenine;  Ap(CH2)pp, alpha,beta-methylene adenosine 5''-triphosphate;  2''-d-3''-AMP, 2''-deoxyadenosine 3''-monophosphate;  3''-AMP, adenosine 3''-monophosphate.	transcription
60167	8	335566	7	NULL	NULL	0	NULL	2''-d-3''-AMP	Chemical		is					2''-deoxyadenosine 3''-monophosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_51_47785_s_341	11602596	The abbreviations used are:   G-protein, heterotrimeric guanine nucleotide-binding protein;  Gsalpha, the alpha subunit of G protein that stimulates adenylyl cyclase;  GTPgammaS, guanosine 5''-(gamma-thio) triphosphate;  THFA, 9-(tetrahydro-2-furyl) adenine;  CPA, 9-(cyclopentyl) adenine;  Ap(CH2)pp, alpha,beta-methylene adenosine 5''-triphosphate;  2''-d-3''-AMP, 2''-deoxyadenosine 3''-monophosphate;  3''-AMP, adenosine 3''-monophosphate.	transcription
60168	9	335566	7	NULL	NULL	0	NULL	3''-AMP	Chemical		is					adenosine 3''-monophosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_51_47785_s_341	11602596	The abbreviations used are:   G-protein, heterotrimeric guanine nucleotide-binding protein;  Gsalpha, the alpha subunit of G protein that stimulates adenylyl cyclase;  GTPgammaS, guanosine 5''-(gamma-thio) triphosphate;  THFA, 9-(tetrahydro-2-furyl) adenine;  CPA, 9-(cyclopentyl) adenine;  Ap(CH2)pp, alpha,beta-methylene adenosine 5''-triphosphate;  2''-d-3''-AMP, 2''-deoxyadenosine 3''-monophosphate;  3''-AMP, adenosine 3''-monophosphate.	transcription
55226	1	335567	5	NULL	NULL	0	NULL	ecto-5''-nucleotidase			is a type of					enzyme					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_48_37572_s_216	10978314	In contrast, Fig.  6 B shows that the formation of adenosine from released adenine nucleotides might be more efficient in AA (30 muM)-treated synaptosomes since the activity of ecto-5''-nucleotidase (the enzyme that forms adenosine from extracellular adenine nucleotides) was greater in AA (30 muM)-treated synaptosomes (2.06  plus-or-minus  0.08 nmol of AMP catabolized per min per mg protein,  n = 5) than in control synaptosomes (0.69  plus-or-minus  0.05 nmol/min/mg of protein,  n = 5).	transcription
55227	2	335567	5	NULL	NULL	0	NULL	adenosine			is formed from					adenine nucleotides		extracellular			NULL	AA treated synaptosomes	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_48_37572_s_216	10978314	In contrast, Fig.  6 B shows that the formation of adenosine from released adenine nucleotides might be more efficient in AA (30 muM)-treated synaptosomes since the activity of ecto-5''-nucleotidase (the enzyme that forms adenosine from extracellular adenine nucleotides) was greater in AA (30 muM)-treated synaptosomes (2.06  plus-or-minus  0.08 nmol of AMP catabolized per min per mg protein,  n = 5) than in control synaptosomes (0.69  plus-or-minus  0.05 nmol/min/mg of protein,  n = 5).	transcription
55228	3	335567	5	NULL	NULL	0	NULL	ecto-5''-nucleotidase			is required for					statement 2					NULL	AA treated synaptosomes	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_48_37572_s_216	10978314	In contrast, Fig.  6 B shows that the formation of adenosine from released adenine nucleotides might be more efficient in AA (30 muM)-treated synaptosomes since the activity of ecto-5''-nucleotidase (the enzyme that forms adenosine from extracellular adenine nucleotides) was greater in AA (30 muM)-treated synaptosomes (2.06  plus-or-minus  0.08 nmol of AMP catabolized per min per mg protein,  n = 5) than in control synaptosomes (0.69  plus-or-minus  0.05 nmol/min/mg of protein,  n = 5).	transcription
55229	4	335567	5	NULL	NULL	0	NULL	adenosine			is formed from					adenine nucleotides		extracellular			NULL	control synaptosomes	0	NULL	NULL	NULL	gw60_jbiolchem_275_48_37572_s_216	10978314	In contrast, Fig.  6 B shows that the formation of adenosine from released adenine nucleotides might be more efficient in AA (30 muM)-treated synaptosomes since the activity of ecto-5''-nucleotidase (the enzyme that forms adenosine from extracellular adenine nucleotides) was greater in AA (30 muM)-treated synaptosomes (2.06  plus-or-minus  0.08 nmol of AMP catabolized per min per mg protein,  n = 5) than in control synaptosomes (0.69  plus-or-minus  0.05 nmol/min/mg of protein,  n = 5).	transcription
55230	5	335567	5	NULL	NULL	0	NULL	ecto-5''-nucleotidase			is required for					statement 4					NULL	control synaptosomes	0	NULL	NULL	NULL	gw60_jbiolchem_275_48_37572_s_216	10978314	In contrast, Fig.  6 B shows that the formation of adenosine from released adenine nucleotides might be more efficient in AA (30 muM)-treated synaptosomes since the activity of ecto-5''-nucleotidase (the enzyme that forms adenosine from extracellular adenine nucleotides) was greater in AA (30 muM)-treated synaptosomes (2.06  plus-or-minus  0.08 nmol of AMP catabolized per min per mg protein,  n = 5) than in control synaptosomes (0.69  plus-or-minus  0.05 nmol/min/mg of protein,  n = 5).	transcription
55231	6	335567	5	NULL	NULL	0	NULL	statement 2			more efficient than					statement 4					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_48_37572_s_216	10978314	In contrast, Fig.  6 B shows that the formation of adenosine from released adenine nucleotides might be more efficient in AA (30 muM)-treated synaptosomes since the activity of ecto-5''-nucleotidase (the enzyme that forms adenosine from extracellular adenine nucleotides) was greater in AA (30 muM)-treated synaptosomes (2.06  plus-or-minus  0.08 nmol of AMP catabolized per min per mg protein,  n = 5) than in control synaptosomes (0.69  plus-or-minus  0.05 nmol/min/mg of protein,  n = 5).	transcription
55232	7	335567	5	NULL	NULL	0	NULL	statement 3			greater activity than					statement 5					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_48_37572_s_216	10978314	In contrast, Fig.  6 B shows that the formation of adenosine from released adenine nucleotides might be more efficient in AA (30 muM)-treated synaptosomes since the activity of ecto-5''-nucleotidase (the enzyme that forms adenosine from extracellular adenine nucleotides) was greater in AA (30 muM)-treated synaptosomes (2.06  plus-or-minus  0.08 nmol of AMP catabolized per min per mg protein,  n = 5) than in control synaptosomes (0.69  plus-or-minus  0.05 nmol/min/mg of protein,  n = 5).	transcription
55233	8	335567	5	NULL	NULL	0	NULL	statement 7			leads to					statement 6					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_48_37572_s_216	10978314	In contrast, Fig.  6 B shows that the formation of adenosine from released adenine nucleotides might be more efficient in AA (30 muM)-treated synaptosomes since the activity of ecto-5''-nucleotidase (the enzyme that forms adenosine from extracellular adenine nucleotides) was greater in AA (30 muM)-treated synaptosomes (2.06  plus-or-minus  0.08 nmol of AMP catabolized per min per mg protein,  n = 5) than in control synaptosomes (0.69  plus-or-minus  0.05 nmol/min/mg of protein,  n = 5).	transcription
60169	1	335567	7	NULL	NULL	0	NULL	adenosine	NucleicAcid		formed from					adenine nucleotides	NucleicAcid	extracellular			NULL	AA treated synaptosomes	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_48_37572_s_216	10978314	In contrast, Fig.  6 B shows that the formation of adenosine from released adenine nucleotides might be more efficient in AA (30 muM)-treated synaptosomes since the activity of ecto-5''-nucleotidase (the enzyme that forms adenosine from extracellular adenine nucleotides) was greater in AA (30 muM)-treated synaptosomes (2.06  plus-or-minus  0.08 nmol of AMP catabolized per min per mg protein,  n = 5) than in control synaptosomes (0.69  plus-or-minus  0.05 nmol/min/mg of protein,  n = 5).	transcription
60233	2	335567	7	NULL	NULL	0	NULL	ecto-5''-nucleotidase	GP		catalyze					statement 1	Process				NULL	AA treated synaptosomes	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_48_37572_s_216	10978314	In contrast, Fig.  6 B shows that the formation of adenosine from released adenine nucleotides might be more efficient in AA (30 muM)-treated synaptosomes since the activity of ecto-5''-nucleotidase (the enzyme that forms adenosine from extracellular adenine nucleotides) was greater in AA (30 muM)-treated synaptosomes (2.06  plus-or-minus  0.08 nmol of AMP catabolized per min per mg protein,  n = 5) than in control synaptosomes (0.69  plus-or-minus  0.05 nmol/min/mg of protein,  n = 5).	transcription
55234	1	335568	5	NULL	NULL	0	NULL	9-(cyclopentyl)adenine			inhibits		selectively			type 5 AC					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_39_40938_s_149	15262973	For comparison, 9-(cyclopentyl)adenine also inhibited type 5 AC in a similarly selective manner as PMC-6 (632 for type 2 AC and 79 for type 3 AC), as already reported by us ( ) and others ( ), although the IC50 value for type 5 AC (3.2 muM) was greater than that of PMC-6 (0.32 muM).	transcription
55235	2	335568	5	NULL	NULL	0	NULL	PMC-6			inhibits		selectively			type 5 AC					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_39_40938_s_149	15262973	For comparison, 9-(cyclopentyl)adenine also inhibited type 5 AC in a similarly selective manner as PMC-6 (632 for type 2 AC and 79 for type 3 AC), as already reported by us ( ) and others ( ), although the IC50 value for type 5 AC (3.2 muM) was greater than that of PMC-6 (0.32 muM).	transcription
60234	1	335568	7	NULL	NULL	0	NULL	9-(cyclopentyl)adenine 	Chemical		inhibit					 type 5 AC	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_39_40938_s_149	15262973	For comparison, 9-(cyclopentyl)adenine also inhibited type 5 AC in a similarly selective manner as PMC-6 (632 for type 2 AC and 79 for type 3 AC), as already reported by us ( ) and others ( ), although the IC50 value for type 5 AC (3.2 muM) was greater than that of PMC-6 (0.32 muM).	transcription
60235	2	335568	7	NULL	NULL	0	NULL	PMC-6	Chemical		inhibit					type 5 AC	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_39_40938_s_149	15262973	For comparison, 9-(cyclopentyl)adenine also inhibited type 5 AC in a similarly selective manner as PMC-6 (632 for type 2 AC and 79 for type 3 AC), as already reported by us ( ) and others ( ), although the IC50 value for type 5 AC (3.2 muM) was greater than that of PMC-6 (0.32 muM).	transcription
60236	3	335568	7	NULL	NULL	0	NULL	statement 1	Process	inhibition of	is similar to					statement 2	Process	inhibition of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_39_40938_s_149	15262973	For comparison, 9-(cyclopentyl)adenine also inhibited type 5 AC in a similarly selective manner as PMC-6 (632 for type 2 AC and 79 for type 3 AC), as already reported by us ( ) and others ( ), although the IC50 value for type 5 AC (3.2 muM) was greater than that of PMC-6 (0.32 muM).	transcription
55236	1	335570	5	NULL	NULL	0	NULL	YPH-A cells		growth of;;prototrophic	requires					uracil					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
55237	2	335570	5	NULL	NULL	0	NULL	YPH-A cells		growth of;;prototrophic	requires					adenine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
55238	3	335570	5	NULL	NULL	0	NULL	YPH-E cells		growth of;;prototrophic	requires					uracil					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
55239	4	335570	5	NULL	NULL	0	NULL	YPH-E cells		growth of;;prototrophic	requires					adenine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
55240	5	335570	5	NULL	NULL	0	NULL	PHS		high concentration of	inhibits					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
55241	6	335570	5	NULL	NULL	0	NULL	PHS		high concentration of	inhibits					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
55242	7	335570	5	NULL	NULL	0	NULL	PHS		high concentration of	inhibits					statement 3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
55243	8	335570	5	NULL	NULL	0	NULL	PHS		high concentration of	inhibits					statement 4					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
55244	9	335570	5	NULL	NULL	0	NULL	proline			is the source of					nitrogen					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
55245	10	335570	5	NULL	NULL	0	NULL	ammonium ions 			is the source of					nitrogen					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
55246	11	335570	5	NULL	NULL	0	NULL	statement 9			is preferred over					statement 10					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
60237	1	335570	7	NULL	NULL	0	NULL	YPH-A cells	Cell	growth of	require					Uracil	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
60238	2	335570	7	NULL	NULL	0	NULL	YPH-A cells	Cell	growth of	require					adenine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
60239	3	335570	7	NULL	NULL	0	NULL	YPH-E cells	Cell	growth of	require					Uracil	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
60240	4	335570	7	NULL	NULL	0	NULL	YPH-E cells	Cell	growth of	require					adenine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
60241	5	335570	7	NULL	NULL	0	NULL	PHS	Chemical		inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
60242	6	335570	7	NULL	NULL	0	NULL	PHS	Chemical		inhibit					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
60243	7	335570	7	NULL	NULL	0	NULL	PHS	Chemical		inhibit					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
60244	8	335570	7	NULL	NULL	0	NULL	PHS	Chemical		inhibit					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
60250	9	335570	7	NULL	NULL	0	NULL	proline	AminoAcid		used as a					nitrogen source	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
60251	10	335570	7	NULL	NULL	0	NULL	Ammonium ions	Chemical		used as a					nitrogen source	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
60252	11	335570	7	NULL	NULL	0	NULL	statement 5	Process		occur upon					statement 9	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
60253	12	335570	7	NULL	NULL	0	NULL	statement 6	Process		occur upon					statement 9	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
60254	13	335570	7	NULL	NULL	0	NULL	statement 7	Process		occur upon					statement 9	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
60255	14	335570	7	NULL	NULL	0	NULL	statement 8	Process		occur upon					statement 9	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
60256	15	335570	7	NULL	NULL	0	NULL	statement 5	Process		occur upon					statement 10	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
60257	16	335570	7	NULL	NULL	0	NULL	statement 6	Process		occur upon					statement 10	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
60258	17	335570	7	NULL	NULL	0	NULL	statement 7	Process		occur upon					statement 10	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
60263	18	335570	7	NULL	NULL	0	NULL	statement 8	Process		occur upon					statement 10	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
60269	19	335570	7	NULL	NULL	0	NULL	statement 11	Process	inhibition of	is more than					statement 15	Process	inhibition of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
60270	20	335570	7	NULL	NULL	0	NULL	statement 12	Process	inhibition of	is more than					statement 16	Process	inhibition of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
60271	21	335570	7	NULL	NULL	0	NULL	statement 13	Process	inhibition of	is more than					statement 17	Process	inhibition of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
60272	22	335570	7	NULL	NULL	0	NULL	statement 14	Process	inhibition of	is more than					statement 18	Process	inhibition of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
60273	23	335570	7	NULL	NULL	0	NULL	YPH-A cell	Cell		is a type of					prototrophic cell	Cell				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
60274	24	335570	7	NULL	NULL	0	NULL	YPH-E cell	Cell		is a type of					prototrophic cell	Cell				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_153	9446592	Growth of prototrophic YPH-A and YPH-E cells requiring uracil and adenine was slightly more inhibited by high concentrations of PHS when proline (Fig.  5 B) rather than ammonium ions were the nitrogen source (Fig.  5 A).	transcription
55247	1	335572	5	NULL	NULL	0	NULL	AFB1 exo-8,9-epoxide			reacts with					adenine bases					NULL		0	NULL	NULL	NULL	gw60_pnas_94_12_6121_s_98	9177180	Because AFB1  exo-8,9-epoxide reacts with adenine bases only 1% as effectively as Gua ( 22), we also investigated the effect of poly d(AT), which is necessarily duplex helical DNA and shown to intercalate AFB1 ( 5); its presence produced a 33% rate enhancement (Fig.  5).	transcription
55248	2	335572	5	NULL	NULL	0	NULL	poly d(AT)			is a type of					duplex helical DNA					NULL		0	NULL	NULL	NULL	gw60_pnas_94_12_6121_s_98	9177180	Because AFB1  exo-8,9-epoxide reacts with adenine bases only 1% as effectively as Gua ( 22), we also investigated the effect of poly d(AT), which is necessarily duplex helical DNA and shown to intercalate AFB1 ( 5); its presence produced a 33% rate enhancement (Fig.  5).	transcription
55249	3	335572	5	NULL	NULL	0	NULL	poly d(AT)			intercalate					AFB1					NULL		0	NULL	NULL	NULL	gw60_pnas_94_12_6121_s_98	9177180	Because AFB1  exo-8,9-epoxide reacts with adenine bases only 1% as effectively as Gua ( 22), we also investigated the effect of poly d(AT), which is necessarily duplex helical DNA and shown to intercalate AFB1 ( 5); its presence produced a 33% rate enhancement (Fig.  5).	transcription
60280	1	335572	7	NULL	NULL	0	NULL	AFB1 exo-8,9-epoxide	Chemical		reacts with					adenine bases	Chemical				NULL		0	NULL	NULL	NULL	gw60_pnas_94_12_6121_s_98	9177180	Because AFB1  exo-8,9-epoxide reacts with adenine bases only 1% as effectively as Gua ( 22), we also investigated the effect of poly d(AT), which is necessarily duplex helical DNA and shown to intercalate AFB1 ( 5); its presence produced a 33% rate enhancement (Fig.  5).	transcription
60283	2	335572	7	NULL	NULL	0	NULL	AFB1 exo-8,9-epoxide	Chemical		reacts with					Gua	Chemical				NULL		0	NULL	NULL	NULL	gw60_pnas_94_12_6121_s_98	9177180	Because AFB1  exo-8,9-epoxide reacts with adenine bases only 1% as effectively as Gua ( 22), we also investigated the effect of poly d(AT), which is necessarily duplex helical DNA and shown to intercalate AFB1 ( 5); its presence produced a 33% rate enhancement (Fig.  5).	transcription
60288	3	335572	7	NULL	NULL	0	NULL	poly d(AT)	NucleicAcid		intercalate					AFB1	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_12_6121_s_98	9177180	Because AFB1  exo-8,9-epoxide reacts with adenine bases only 1% as effectively as Gua ( 22), we also investigated the effect of poly d(AT), which is necessarily duplex helical DNA and shown to intercalate AFB1 ( 5); its presence produced a 33% rate enhancement (Fig.  5).	transcription
60289	4	335572	7	NULL	NULL	0	NULL	poly d(AT)	NucleicAcid		is a type of					duplex helical DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_pnas_94_12_6121_s_98	9177180	Because AFB1  exo-8,9-epoxide reacts with adenine bases only 1% as effectively as Gua ( 22), we also investigated the effect of poly d(AT), which is necessarily duplex helical DNA and shown to intercalate AFB1 ( 5); its presence produced a 33% rate enhancement (Fig.  5).	transcription
55250	1	335573	5	NULL	NULL	0	NULL	Choline			does not affect					yeast		vitality of			NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_84	10359089	Choline did not affect yeast vitality or the electrochemical gradient, since the transport of [U-14]adenine by endogenous yeast H+-cotransport systems [  24] was uninhibited by the presence of 0, 5 or 25 mM choline (783 plus-or-minus 97, 778 plus-or-minus 63 and 800 plus-or-minus 34 nmol adenine min~1 g~1 yeast DW).	transcription
55251	2	335573	5	NULL	NULL	0	NULL	[U-14]adenine			is transported by					H+-cotransport systems		endogenous;;yeast			NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_84	10359089	Choline did not affect yeast vitality or the electrochemical gradient, since the transport of [U-14]adenine by endogenous yeast H+-cotransport systems [  24] was uninhibited by the presence of 0, 5 or 25 mM choline (783 plus-or-minus 97, 778 plus-or-minus 63 and 800 plus-or-minus 34 nmol adenine min~1 g~1 yeast DW).	transcription
55252	3	335573	5	NULL	NULL	0	NULL	choline		presence of	inhibits					statement 2					NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_84	10359089	Choline did not affect yeast vitality or the electrochemical gradient, since the transport of [U-14]adenine by endogenous yeast H+-cotransport systems [  24] was uninhibited by the presence of 0, 5 or 25 mM choline (783 plus-or-minus 97, 778 plus-or-minus 63 and 800 plus-or-minus 34 nmol adenine min~1 g~1 yeast DW).	transcription
60290	1	335573	7	NULL	NULL	0	NULL	Choline	Chemical		does not affect					yeast vitality	Organism				NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_84	10359089	Choline did not affect yeast vitality or the electrochemical gradient, since the transport of [U-14]adenine by endogenous yeast H+-cotransport systems [  24] was uninhibited by the presence of 0, 5 or 25 mM choline (783 plus-or-minus 97, 778 plus-or-minus 63 and 800 plus-or-minus 34 nmol adenine min~1 g~1 yeast DW).	transcription
60291	2	335573	7	NULL	NULL	0	NULL	Choline	Chemical		does not affect					electrochemical gradient	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_450_3_280_s_84	10359089	Choline did not affect yeast vitality or the electrochemical gradient, since the transport of [U-14]adenine by endogenous yeast H+-cotransport systems [  24] was uninhibited by the presence of 0, 5 or 25 mM choline (783 plus-or-minus 97, 778 plus-or-minus 63 and 800 plus-or-minus 34 nmol adenine min~1 g~1 yeast DW).	transcription
60292	3	335573	7	NULL	NULL	0	NULL	H+-cotransport system	Process	yeast;;endogenous	transport					[U-14]adenine	Chemical				NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_84	10359089	Choline did not affect yeast vitality or the electrochemical gradient, since the transport of [U-14]adenine by endogenous yeast H+-cotransport systems [  24] was uninhibited by the presence of 0, 5 or 25 mM choline (783 plus-or-minus 97, 778 plus-or-minus 63 and 800 plus-or-minus 34 nmol adenine min~1 g~1 yeast DW).	transcription
60293	4	335573	7	NULL	NULL	0	NULL	Choline	Chemical		does not inhibit					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_84	10359089	Choline did not affect yeast vitality or the electrochemical gradient, since the transport of [U-14]adenine by endogenous yeast H+-cotransport systems [  24] was uninhibited by the presence of 0, 5 or 25 mM choline (783 plus-or-minus 97, 778 plus-or-minus 63 and 800 plus-or-minus 34 nmol adenine min~1 g~1 yeast DW).	transcription
55253	1	335575	5	NULL	NULL	0	NULL	MYH			catalyzes					adenine base 		excision of			NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_32_19_5928_s_77	15531653	Adenine base excision catalyzed by MYH and APE1   The reaction mixture (20 mul) contained 50 mM Tris - HCl (pH 7.5), 5 mM MgCl2, 5 mM DTT, 50 mug/ml BSA, 1 nM 5''-labeled 40mer duplex DNA and MYH (0, 2.5, 5 or 10 nM) and was incubated at 37 degrees C for 15 min followed by incubation with APE1 (0, 10 or 50 nM) in the presence of 150 mM KCl at 37 degrees C for 15 min ( Figure 5).	transcription
55254	2	335575	5	NULL	NULL	0	NULL	APE1			catalyzes					adenine base		excision of			NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_32_19_5928_s_77	15531653	Adenine base excision catalyzed by MYH and APE1   The reaction mixture (20 mul) contained 50 mM Tris - HCl (pH 7.5), 5 mM MgCl2, 5 mM DTT, 50 mug/ml BSA, 1 nM 5''-labeled 40mer duplex DNA and MYH (0, 2.5, 5 or 10 nM) and was incubated at 37 degrees C for 15 min followed by incubation with APE1 (0, 10 or 50 nM) in the presence of 150 mM KCl at 37 degrees C for 15 min ( Figure 5).	transcription
60294	1	335575	7	NULL	NULL	0	NULL	Adenine base	Chemical	excision of	catalyzed by					MYH	GP				NULL		0	NULL	NULL	NULL	gw70_nucleicacidsres_32_19_5928_s_77	15531653	Adenine base excision catalyzed by MYH and APE1   The reaction mixture (20 mul) contained 50 mM Tris - HCl (pH 7.5), 5 mM MgCl2, 5 mM DTT, 50 mug/ml BSA, 1 nM 5''-labeled 40mer duplex DNA and MYH (0, 2.5, 5 or 10 nM) and was incubated at 37 degrees C for 15 min followed by incubation with APE1 (0, 10 or 50 nM) in the presence of 150 mM KCl at 37 degrees C for 15 min ( Figure 5).	transcription
60295	2	335575	7	NULL	NULL	0	NULL	Adenine base	Chemical	excision of	catalyzed by					APE1	GP				NULL		NULL	NULL	NULL	NULL	gw70_nucleicacidsres_32_19_5928_s_77	15531653	Adenine base excision catalyzed by MYH and APE1   The reaction mixture (20 mul) contained 50 mM Tris - HCl (pH 7.5), 5 mM MgCl2, 5 mM DTT, 50 mug/ml BSA, 1 nM 5''-labeled 40mer duplex DNA and MYH (0, 2.5, 5 or 10 nM) and was incubated at 37 degrees C for 15 min followed by incubation with APE1 (0, 10 or 50 nM) in the presence of 150 mM KCl at 37 degrees C for 15 min ( Figure 5).	transcription
60296	1	335576	7	NULL	NULL	0	NULL	 IRF-3	GP		bind								Arg 81	 3' site opposite guanine	NULL		0	NULL	NULL	NULL	gw70_embo_23_22_4384_s_95	15510218	We find that IRF-3 binds the 3' site in the standard fashion, with  Arg 81 opposite the guanine ( Figure 2), but it binds the 5' site 1 bp 'out of phase'', with Arg 81 opposite  the first adenine, thus preserving the canonical 2 bp intersite spacing, at the expense  of the usually conserved contact of Arg 81 with guanine.	transcription
60297	2	335576	7	NULL	NULL	0	NULL	IRF-3	GP		bind								Arg 81	5' site opposite first adenine	NULL		0	NULL	NULL	NULL	gw70_embo_23_22_4384_s_95	15510218	We find that IRF-3 binds the 3' site in the standard fashion, with  Arg 81 opposite the guanine ( Figure 2), but it binds the 5' site 1 bp 'out of phase'', with Arg 81 opposite  the first adenine, thus preserving the canonical 2 bp intersite spacing, at the expense  of the usually conserved contact of Arg 81 with guanine.	transcription
60298	3	335576	7	NULL	NULL	0	NULL	statement 2	Process		occurs					out of phase	Process				NULL		0	NULL	NULL	NULL	gw70_embo_23_22_4384_s_95	15510218	We find that IRF-3 binds the 3' site in the standard fashion, with  Arg 81 opposite the guanine ( Figure 2), but it binds the 5' site 1 bp 'out of phase'', with Arg 81 opposite  the first adenine, thus preserving the canonical 2 bp intersite spacing, at the expense  of the usually conserved contact of Arg 81 with guanine.	transcription
60299	4	335576	7	NULL	NULL	0	NULL	statement 3	Process		preserves					 intersite spacing	QuantityOrMeasure				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_22_4384_s_95	15510218	We find that IRF-3 binds the 3' site in the standard fashion, with  Arg 81 opposite the guanine ( Figure 2), but it binds the 5' site 1 bp 'out of phase'', with Arg 81 opposite  the first adenine, thus preserving the canonical 2 bp intersite spacing, at the expense  of the usually conserved contact of Arg 81 with guanine.	transcription
60300	5	335576	7	NULL	NULL	0	NULL				contact with		conserved	Arg 81		guanine	Chemical				NULL		0	NULL	NULL	NULL	gw70_embo_23_22_4384_s_95	15510218	We find that IRF-3 binds the 3' site in the standard fashion, with  Arg 81 opposite the guanine ( Figure 2), but it binds the 5' site 1 bp 'out of phase'', with Arg 81 opposite  the first adenine, thus preserving the canonical 2 bp intersite spacing, at the expense  of the usually conserved contact of Arg 81 with guanine.	transcription
60301	6	335576	7	NULL	NULL	0	NULL	statement 4	Process		at the expense of					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_embo_23_22_4384_s_95	15510218	We find that IRF-3 binds the 3' site in the standard fashion, with  Arg 81 opposite the guanine ( Figure 2), but it binds the 5' site 1 bp 'out of phase'', with Arg 81 opposite  the first adenine, thus preserving the canonical 2 bp intersite spacing, at the expense  of the usually conserved contact of Arg 81 with guanine.	transcription
55255	1	335577	5	NULL	NULL	0	NULL	ATP			is a type of					adenine-based nucleotides					NULL		0	NULL	NULL	NULL	gw70_intjdevneurosci_19_4_395_s_281	11378300	In  cultures of rat astrocytes, exogenous GTP substantially increases the extracellular  levels of adenine-based nucleotides (mainly ATP and AMP) from rat astrocytes, an  effect at least in part ascribable to the blockade of 5 -ectonucleotidase (   Rathbone et al., 1998b , 1999).	transcription
55256	2	335577	5	NULL	NULL	0	NULL	AMP			is a type of					adenine-based nucleotides					NULL		0	NULL	NULL	NULL	gw70_intjdevneurosci_19_4_395_s_281	11378300	In  cultures of rat astrocytes, exogenous GTP substantially increases the extracellular  levels of adenine-based nucleotides (mainly ATP and AMP) from rat astrocytes, an  effect at least in part ascribable to the blockade of 5 -ectonucleotidase (   Rathbone et al., 1998b , 1999).	transcription
55257	3	335577	5	NULL	NULL	0	NULL	GTP		exogenous	increases		substantially			ATP		extracellular levels of			NULL	cultures of rat astrocytes	0	NULL	NULL	NULL	gw70_intjdevneurosci_19_4_395_s_281	11378300	In  cultures of rat astrocytes, exogenous GTP substantially increases the extracellular  levels of adenine-based nucleotides (mainly ATP and AMP) from rat astrocytes, an  effect at least in part ascribable to the blockade of 5 -ectonucleotidase (   Rathbone et al., 1998b , 1999).	transcription
55258	4	335577	5	NULL	NULL	0	NULL	GTP		exogenous	increases		substantially			AMP		extracellular levels of			NULL	cultures of rat astrocytes	0	NULL	NULL	NULL	gw70_intjdevneurosci_19_4_395_s_281	11378300	In  cultures of rat astrocytes, exogenous GTP substantially increases the extracellular  levels of adenine-based nucleotides (mainly ATP and AMP) from rat astrocytes, an  effect at least in part ascribable to the blockade of 5 -ectonucleotidase (   Rathbone et al., 1998b , 1999).	transcription
55259	5	335577	5	NULL	NULL	0	NULL	statement 3			ascribable to		partly			5 -ectonucleotidase		blockade of			NULL	cultures of rat astrocytes	NULL	NULL	NULL	NULL	gw70_intjdevneurosci_19_4_395_s_281	11378300	In  cultures of rat astrocytes, exogenous GTP substantially increases the extracellular  levels of adenine-based nucleotides (mainly ATP and AMP) from rat astrocytes, an  effect at least in part ascribable to the blockade of 5 -ectonucleotidase (   Rathbone et al., 1998b , 1999).	transcription
55260	6	335577	5	NULL	NULL	0	NULL	statement 4			ascribable to		partly			5 -ectonucleotidase		blockade of			NULL	cultures of rat astrocytes	NULL	NULL	NULL	NULL	gw70_intjdevneurosci_19_4_395_s_281	11378300	In  cultures of rat astrocytes, exogenous GTP substantially increases the extracellular  levels of adenine-based nucleotides (mainly ATP and AMP) from rat astrocytes, an  effect at least in part ascribable to the blockade of 5 -ectonucleotidase (   Rathbone et al., 1998b , 1999).	transcription
60302	1	335577	7	NULL	NULL	0	NULL	 GTP	Chemical	exogenous	increase					ATP	Chemical	extracellular levels of			NULL	rat astrocytes	0	NULL	NULL	NULL	gw70_intjdevneurosci_19_4_395_s_281	11378300	In  cultures of rat astrocytes, exogenous GTP substantially increases the extracellular  levels of adenine-based nucleotides (mainly ATP and AMP) from rat astrocytes, an  effect at least in part ascribable to the blockade of 5 -ectonucleotidase (   Rathbone et al., 1998b , 1999).	transcription
60303	2	335577	7	NULL	NULL	0	NULL	GTP	Chemical	exogenous	increase					AMP	Chemical	extracellular levels of			NULL	rat astrocytes	NULL	NULL	NULL	NULL	gw70_intjdevneurosci_19_4_395_s_281	11378300	In  cultures of rat astrocytes, exogenous GTP substantially increases the extracellular  levels of adenine-based nucleotides (mainly ATP and AMP) from rat astrocytes, an  effect at least in part ascribable to the blockade of 5 -ectonucleotidase (   Rathbone et al., 1998b , 1999).	transcription
60304	3	335577	7	NULL	NULL	0	NULL	statement 1	Process		ascribable to		partly			5 -ectonucleotidase	GP	blockade of			NULL		0	NULL	NULL	NULL	gw70_intjdevneurosci_19_4_395_s_281	11378300	In  cultures of rat astrocytes, exogenous GTP substantially increases the extracellular  levels of adenine-based nucleotides (mainly ATP and AMP) from rat astrocytes, an  effect at least in part ascribable to the blockade of 5 -ectonucleotidase (   Rathbone et al., 1998b , 1999).	transcription
60305	4	335577	7	NULL	NULL	0	NULL	statement 2	Process		ascribable to		partly			5 -ectonucleotidase	GP	blockade of			NULL		NULL	NULL	NULL	NULL	gw70_intjdevneurosci_19_4_395_s_281	11378300	In  cultures of rat astrocytes, exogenous GTP substantially increases the extracellular  levels of adenine-based nucleotides (mainly ATP and AMP) from rat astrocytes, an  effect at least in part ascribable to the blockade of 5 -ectonucleotidase (   Rathbone et al., 1998b , 1999).	transcription
60306	5	335577	7	NULL	NULL	0	NULL	ATP	Chemical		is a type of					adenine-based nucleotide	Chemical				NULL		0	NULL	NULL	NULL	gw70_intjdevneurosci_19_4_395_s_281	11378300	In  cultures of rat astrocytes, exogenous GTP substantially increases the extracellular  levels of adenine-based nucleotides (mainly ATP and AMP) from rat astrocytes, an  effect at least in part ascribable to the blockade of 5 -ectonucleotidase (   Rathbone et al., 1998b , 1999).	transcription
60307	6	335577	7	NULL	NULL	0	NULL	AMP	Chemical		is a type of					adenine-based nucleotide	Chemical				NULL		0	NULL	NULL	NULL	gw70_intjdevneurosci_19_4_395_s_281	11378300	In  cultures of rat astrocytes, exogenous GTP substantially increases the extracellular  levels of adenine-based nucleotides (mainly ATP and AMP) from rat astrocytes, an  effect at least in part ascribable to the blockade of 5 -ectonucleotidase (   Rathbone et al., 1998b , 1999).	transcription
55261	1	335578	5	NULL	NULL	0	NULL	HDAC 1			is related to					RPD3		yeast			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
55262	2	335578	5	NULL	NULL	0	NULL	HDAC 2			is related to					RPD3		yeast			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
55263	3	335578	5	NULL	NULL	0	NULL	HDAC 3			is related to					RPD3		yeast			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
55264	4	335578	5	NULL	NULL	0	NULL	HDAC 8			is related to					RPD3		yeast			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
55265	5	335578	5	NULL	NULL	0	NULL	HDAC 4			is related to					Had1					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
55266	6	335578	5	NULL	NULL	0	NULL	HDAC 5			is related to					Had1					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
55267	7	335578	5	NULL	NULL	0	NULL	HDAC 6			is related to					Had1					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
55268	8	335578	5	NULL	NULL	0	NULL	HDAC 7			is related to					Had1					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
55269	9	335578	5	NULL	NULL	0	NULL	class III HDACs			is related to					Sir2 family					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
55270	10	335578	5	NULL	NULL	0	NULL	Sir2 family		activity of	is dependent on					nicotinamide-adenine-dinucleotide					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
55271	11	335578	5	NULL	NULL	0	NULL	HDAC 1			is a type of					Class 1 HDAC					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
55272	12	335578	5	NULL	NULL	0	NULL	HDAC 2			is a type of					Class 1 HDAC					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
55273	13	335578	5	NULL	NULL	0	NULL	HDAC 3			is a type of					Class 1 HDAC					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
55274	14	335578	5	NULL	NULL	0	NULL	HDAC 8			is a type of					Class 1 HDAC					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
55275	15	335578	5	NULL	NULL	0	NULL	HDAC 4			is a type of					class II HDAC					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
55276	16	335578	5	NULL	NULL	0	NULL	HDAC 5			is a type of					class II HDAC					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
55277	17	335578	5	NULL	NULL	0	NULL	HDAC 6			is a type of					class II HDAC					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
55278	18	335578	5	NULL	NULL	0	NULL	HDAC 7			is a type of					class II HDAC					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
60308	1	335578	7	NULL	NULL	0	NULL	HDAC 1	GP		is related to					RPD3	GP	yeast			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
60309	2	335578	7	NULL	NULL	0	NULL	HDAC 2	GP		is related to					RPD3	GP	yeast			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
60310	3	335578	7	NULL	NULL	0	NULL	HDAC 3	GP		is related to					RPD3	GP	yeast			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
60311	4	335578	7	NULL	NULL	0	NULL	HDAC 8	GP		is related to					RPD3	GP	yeast			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
60312	5	335578	7	NULL	NULL	0	NULL	HDAC 4	GP		is related to					Had1	GP				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
60313	6	335578	7	NULL	NULL	0	NULL	HDAC 5	GP		is related to					Had1	GP				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
60314	7	335578	7	NULL	NULL	0	NULL	HDAC 6	GP		is related to					Had1	GP				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
60315	8	335578	7	NULL	NULL	0	NULL	HDAC 7	GP		is related to					Had1	GP				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
60316	9	335578	7	NULL	NULL	0	NULL	class III HDAC 	GP		is related to					 Sir2 family	GP				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
60317	10	335578	7	NULL	NULL	0	NULL	Sir2 family	GP	activity of	depends on					nicotinamide-adenine-dinucleotide	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
60318	11	335578	7	NULL	NULL	0	NULL	HDAC 1	GP		is a type of					Class I molecule	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
60319	12	335578	7	NULL	NULL	0	NULL	HDAC 2	GP		is a type of					Class I molecule	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
60320	13	335578	7	NULL	NULL	0	NULL	HDAC 3	GP		is a type of					Class I molecule	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
60321	14	335578	7	NULL	NULL	0	NULL	HDAC 8	GP		is a type of					Class I molecule	GP				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
60322	15	335578	7	NULL	NULL	0	NULL	HDAC 4	GP		is a type of					Class II molecule	GP				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
60323	16	335578	7	NULL	NULL	0	NULL	HDAC 5	GP		is a type of					Class II molecule	GP				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
60324	17	335578	7	NULL	NULL	0	NULL	HDAC 6	GP		is a type of					Class II molecule	GP				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
60325	18	335578	7	NULL	NULL	0	NULL	HDAC 7	GP		is a type of					Class II molecule	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1677_1_30_s_204	15020043	Class 1 (HDAC 1, 2, 3  and 8) are related to yeast RPD3, class II (HDAC 4, 5, 6 and 7) are related to Had1  and class III HDACs are related to Sir2 family whose activity depends on nicotinamide-adenine-dinucleotide  [  137].	transcription
56504	1	335579	5	NULL	NULL	0	NULL	adenine base		phosphates 5' to alkylated	interacts with					AlkBs		eubacterial	Thr 51;;Tyr 76 ;;Arg 161		NULL		0	NULL	NULL	NULL	gw70_nature_439_7078_879_s_60	16482161	The nucleotide backbone is bound in a cooperative hydrogen-bonding (H-bonding) network  in which the two phosphates 5' to the alkylated adenine base interact with Thr  51, Tyr 76 and Arg 161 ( Fig. 2b), which are invariant in eubacterial AlkBs ( Supplementary Fig. S2A).	transcription
60342	1	335579	7	NULL	NULL	0	NULL	nucleotide	NucleicAcid	binding of backbone of	occur as a 					H-bonding network	Process	cooperative			NULL		NULL	NULL	NULL	NULL	gw70_nature_439_7078_879_s_60	16482161	The nucleotide backbone is bound in a cooperative hydrogen-bonding (H-bonding) network  in which the two phosphates 5' to the alkylated adenine base interact with Thr  51, Tyr 76 and Arg 161 ( Fig. 2b), which are invariant in eubacterial AlkBs ( Supplementary Fig. S2A).	transcription
60343	2	335579	7	NULL	NULL	0	NULL	adenine base	Chemical	alkylated	interacts with				two phosphates 5' 				Thr51		NULL	eubacterial AlkBs 	0	NULL	NULL	NULL	gw70_nature_439_7078_879_s_60	16482161	The nucleotide backbone is bound in a cooperative hydrogen-bonding (H-bonding) network  in which the two phosphates 5' to the alkylated adenine base interact with Thr  51, Tyr 76 and Arg 161 ( Fig. 2b), which are invariant in eubacterial AlkBs ( Supplementary Fig. S2A).	transcription
60344	3	335579	7	NULL	NULL	0	NULL	adenine base	Chemical	alkylated	interacts with				two phosphates 5'				Tyr 76		NULL	eubacterial AlkBs	NULL	NULL	NULL	NULL	gw70_nature_439_7078_879_s_60	16482161	The nucleotide backbone is bound in a cooperative hydrogen-bonding (H-bonding) network  in which the two phosphates 5' to the alkylated adenine base interact with Thr  51, Tyr 76 and Arg 161 ( Fig. 2b), which are invariant in eubacterial AlkBs ( Supplementary Fig. S2A).	transcription
60345	4	335579	7	NULL	NULL	0	NULL	adenine base	Chemical	alkylated	interacts with				two phosphates 5'				Arg 161		NULL	eubacterial AlkBs	0	NULL	NULL	NULL	gw70_nature_439_7078_879_s_60	16482161	The nucleotide backbone is bound in a cooperative hydrogen-bonding (H-bonding) network  in which the two phosphates 5' to the alkylated adenine base interact with Thr  51, Tyr 76 and Arg 161 ( Fig. 2b), which are invariant in eubacterial AlkBs ( Supplementary Fig. S2A).	transcription
60346	5	335579	7	NULL	NULL	0	NULL	statement 2	Process		occur as					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_nature_439_7078_879_s_60	16482161	The nucleotide backbone is bound in a cooperative hydrogen-bonding (H-bonding) network  in which the two phosphates 5' to the alkylated adenine base interact with Thr  51, Tyr 76 and Arg 161 ( Fig. 2b), which are invariant in eubacterial AlkBs ( Supplementary Fig. S2A).	transcription
60347	6	335579	7	NULL	NULL	0	NULL	statement 3	Process		occur as					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_nature_439_7078_879_s_60	16482161	The nucleotide backbone is bound in a cooperative hydrogen-bonding (H-bonding) network  in which the two phosphates 5' to the alkylated adenine base interact with Thr  51, Tyr 76 and Arg 161 ( Fig. 2b), which are invariant in eubacterial AlkBs ( Supplementary Fig. S2A).	transcription
60348	7	335579	7	NULL	NULL	0	NULL	statement 4	Process		occur as					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_nature_439_7078_879_s_60	16482161	The nucleotide backbone is bound in a cooperative hydrogen-bonding (H-bonding) network  in which the two phosphates 5' to the alkylated adenine base interact with Thr  51, Tyr 76 and Arg 161 ( Fig. 2b), which are invariant in eubacterial AlkBs ( Supplementary Fig. S2A).	transcription
60349	8	335579	7	NULL	NULL	0	NULL	H-bonding	Process		is					hydrogen-bonding	Process				NULL		NULL	NULL	NULL	NULL	gw70_nature_439_7078_879_s_60	16482161	The nucleotide backbone is bound in a cooperative hydrogen-bonding (H-bonding) network  in which the two phosphates 5' to the alkylated adenine base interact with Thr  51, Tyr 76 and Arg 161 ( Fig. 2b), which are invariant in eubacterial AlkBs ( Supplementary Fig. S2A).	transcription
55296	1	335580	5	NULL	NULL	0	NULL	ade2 cells			harbor					AtENT1		coding sequences of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35732_s_242	12810710	After inducing the expression of the cloned sequences by  galactose, the  ade2 cells harboring AtENT1 or AtENT3 coding sequences  could grow in the presence of 150 muM adenosine  ( Fig. 5 and data not shown),  indicating that adenine dependence of the  ade2 cells was rescued by  adenosine transport activities of the proteins expressed from the cloned  sequences in the four expression constructs.	transcription
55297	2	335580	5	NULL	NULL	0	NULL	ade2 cells			harbor					AtENT3		coding sequences of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35732_s_242	12810710	After inducing the expression of the cloned sequences by  galactose, the  ade2 cells harboring AtENT1 or AtENT3 coding sequences  could grow in the presence of 150 muM adenosine  ( Fig. 5 and data not shown),  indicating that adenine dependence of the  ade2 cells was rescued by  adenosine transport activities of the proteins expressed from the cloned  sequences in the four expression constructs.	transcription
55298	3	335580	5	NULL	NULL	0	NULL	statement 1			grows					adenosine		in the presence of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_37_35732_s_242	12810710	After inducing the expression of the cloned sequences by  galactose, the  ade2 cells harboring AtENT1 or AtENT3 coding sequences  could grow in the presence of 150 muM adenosine  ( Fig. 5 and data not shown),  indicating that adenine dependence of the  ade2 cells was rescued by  adenosine transport activities of the proteins expressed from the cloned  sequences in the four expression constructs.	transcription
55299	4	335580	5	NULL	NULL	0	NULL	statement 2			grows					adenosine		in the presence of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35732_s_242	12810710	After inducing the expression of the cloned sequences by  galactose, the  ade2 cells harboring AtENT1 or AtENT3 coding sequences  could grow in the presence of 150 muM adenosine  ( Fig. 5 and data not shown),  indicating that adenine dependence of the  ade2 cells was rescued by  adenosine transport activities of the proteins expressed from the cloned  sequences in the four expression constructs.	transcription
55300	5	335580	5	NULL	NULL	0	NULL	ade2 cells			is dependent on					adenine					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35732_s_242	12810710	After inducing the expression of the cloned sequences by  galactose, the  ade2 cells harboring AtENT1 or AtENT3 coding sequences  could grow in the presence of 150 muM adenosine  ( Fig. 5 and data not shown),  indicating that adenine dependence of the  ade2 cells was rescued by  adenosine transport activities of the proteins expressed from the cloned  sequences in the four expression constructs.	transcription
55301	6	335580	5	NULL	NULL	0	NULL	proteins		adenosine transport activities of;;expressed	rescues					statement 5					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35732_s_242	12810710	After inducing the expression of the cloned sequences by  galactose, the  ade2 cells harboring AtENT1 or AtENT3 coding sequences  could grow in the presence of 150 muM adenosine  ( Fig. 5 and data not shown),  indicating that adenine dependence of the  ade2 cells was rescued by  adenosine transport activities of the proteins expressed from the cloned  sequences in the four expression constructs.	transcription
60350	1	335580	7	NULL	NULL	0	NULL	ade2 cells	Cell		depend on					adenine	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_37_35732_s_242	12810710	After inducing the expression of the cloned sequences by  galactose, the  ade2 cells harboring AtENT1 or AtENT3 coding sequences  could grow in the presence of 150 muM adenosine  ( Fig. 5 and data not shown),  indicating that adenine dependence of the  ade2 cells was rescued by  adenosine transport activities of the proteins expressed from the cloned  sequences in the four expression constructs.	transcription
60351	1	335581	7	NULL	NULL	0	NULL	ROR 	GP		bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1494_3_236_s_85	11121580	Because the DNA-binding affinities of ROR  and ROR  reportedly depend on sequences 5' of the consensus half site [ 2,  3,  11 and  16], the ROREs contained a thymine at position -1 and an adenine at position -4 of the nuclear receptor half site.	transcription
60352	2	335581	7	NULL	NULL	0	NULL	statement 1	Process		depend on									sequences 5' of the consensus half site 	NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1494_3_236_s_85	11121580	Because the DNA-binding affinities of ROR  and ROR  reportedly depend on sequences 5' of the consensus half site [ 2,  3,  11 and  16], the ROREs contained a thymine at position -1 and an adenine at position -4 of the nuclear receptor half site.	transcription
60353	3	335581	7	NULL	NULL	0	NULL	statement 1	Process		depend on					 nuclear receptor 	GP			ROREs containing  thymine at position -1 at half site	NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1494_3_236_s_85	11121580	Because the DNA-binding affinities of ROR  and ROR  reportedly depend on sequences 5' of the consensus half site [ 2,  3,  11 and  16], the ROREs contained a thymine at position -1 and an adenine at position -4 of the nuclear receptor half site.	transcription
60354	4	335581	7	NULL	NULL	0	NULL	statement 1	Process		depend on					nuclear receptor	GP			ROREs containing adenine at position -4 at half site	NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1494_3_236_s_85	11121580	Because the DNA-binding affinities of ROR  and ROR  reportedly depend on sequences 5' of the consensus half site [ 2,  3,  11 and  16], the ROREs contained a thymine at position -1 and an adenine at position -4 of the nuclear receptor half site.	transcription
55304	1	335582	5	NULL	NULL	0	NULL	NifL			bind					adenine nucleotides					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1594_2_243_s_212	11904220	We obtained strong evidence that (i) NifL is able to bind and hydrolyze adenine nucleotides at significant rates (  Fig. 2,  Fig. 3,  Fig. 4 and  Fig. 5), and (ii) the presence of ATP or ADP prior to open complex formation stimulates NifL inhibition of NifA transcriptional activity in vitro (  Fig. 1).	transcription
55305	2	335582	5	NULL	NULL	0	NULL	statement 1			hydrolyze					adenine nucleotides					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1594_2_243_s_212	11904220	We obtained strong evidence that (i) NifL is able to bind and hydrolyze adenine nucleotides at significant rates (  Fig. 2,  Fig. 3,  Fig. 4 and  Fig. 5), and (ii) the presence of ATP or ADP prior to open complex formation stimulates NifL inhibition of NifA transcriptional activity in vitro (  Fig. 1).	transcription
55307	3	335582	5	NULL	NULL	0	NULL	NifL			inhibits					NifA		transcriptional activity of			NULL	in vitro	0	NULL	NULL	NULL	gw60_biochimbiophysacta_1594_2_243_s_212	11904220	We obtained strong evidence that (i) NifL is able to bind and hydrolyze adenine nucleotides at significant rates (  Fig. 2,  Fig. 3,  Fig. 4 and  Fig. 5), and (ii) the presence of ATP or ADP prior to open complex formation stimulates NifL inhibition of NifA transcriptional activity in vitro (  Fig. 1).	transcription
55308	4	335582	5	NULL	NULL	0	NULL	ATP		presence of	stimulates					statement 3					NULL	in vitro	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1594_2_243_s_212	11904220	We obtained strong evidence that (i) NifL is able to bind and hydrolyze adenine nucleotides at significant rates (  Fig. 2,  Fig. 3,  Fig. 4 and  Fig. 5), and (ii) the presence of ATP or ADP prior to open complex formation stimulates NifL inhibition of NifA transcriptional activity in vitro (  Fig. 1).	transcription
55310	5	335582	5	NULL	NULL	0	NULL	statement 4			occurs prior to					open complex		formation of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1594_2_243_s_212	11904220	We obtained strong evidence that (i) NifL is able to bind and hydrolyze adenine nucleotides at significant rates (  Fig. 2,  Fig. 3,  Fig. 4 and  Fig. 5), and (ii) the presence of ATP or ADP prior to open complex formation stimulates NifL inhibition of NifA transcriptional activity in vitro (  Fig. 1).	transcription
55312	6	335582	5	NULL	NULL	0	NULL	ADP		presence of	stimulates					statement 3					NULL	in vitro	0	NULL	NULL	NULL	gw60_biochimbiophysacta_1594_2_243_s_212	11904220	We obtained strong evidence that (i) NifL is able to bind and hydrolyze adenine nucleotides at significant rates (  Fig. 2,  Fig. 3,  Fig. 4 and  Fig. 5), and (ii) the presence of ATP or ADP prior to open complex formation stimulates NifL inhibition of NifA transcriptional activity in vitro (  Fig. 1).	transcription
55313	7	335582	5	NULL	NULL	0	NULL	statement 6			occurs prior to					open complex		formation of			NULL	in vitro	0	NULL	NULL	NULL	gw60_biochimbiophysacta_1594_2_243_s_212	11904220	We obtained strong evidence that (i) NifL is able to bind and hydrolyze adenine nucleotides at significant rates (  Fig. 2,  Fig. 3,  Fig. 4 and  Fig. 5), and (ii) the presence of ATP or ADP prior to open complex formation stimulates NifL inhibition of NifA transcriptional activity in vitro (  Fig. 1).	transcription
60355	1	335582	7	NULL	NULL	0	NULL	NifL	GP		bind					adenine nucleotides	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1594_2_243_s_212	11904220	We obtained strong evidence that (i) NifL is able to bind and hydrolyze adenine nucleotides at significant rates (  Fig. 2,  Fig. 3,  Fig. 4 and  Fig. 5), and (ii) the presence of ATP or ADP prior to open complex formation stimulates NifL inhibition of NifA transcriptional activity in vitro (  Fig. 1).	transcription
60356	2	335582	7	NULL	NULL	0	NULL	statement 1	Process		hydrolyze					adenine nucleotides	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1594_2_243_s_212	11904220	We obtained strong evidence that (i) NifL is able to bind and hydrolyze adenine nucleotides at significant rates (  Fig. 2,  Fig. 3,  Fig. 4 and  Fig. 5), and (ii) the presence of ATP or ADP prior to open complex formation stimulates NifL inhibition of NifA transcriptional activity in vitro (  Fig. 1).	transcription
60357	3	335582	7	NULL	NULL	0	NULL	NifL	GP		inhibit					NifA 	GP	transcriptional activity of			NULL	in vitro	0	NULL	NULL	NULL	gw60_biochimbiophysacta_1594_2_243_s_212	11904220	We obtained strong evidence that (i) NifL is able to bind and hydrolyze adenine nucleotides at significant rates (  Fig. 2,  Fig. 3,  Fig. 4 and  Fig. 5), and (ii) the presence of ATP or ADP prior to open complex formation stimulates NifL inhibition of NifA transcriptional activity in vitro (  Fig. 1).	transcription
60358	4	335582	7	NULL	NULL	0	NULL	ATP	Chemical	presence of	stimulate					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1594_2_243_s_212	11904220	We obtained strong evidence that (i) NifL is able to bind and hydrolyze adenine nucleotides at significant rates (  Fig. 2,  Fig. 3,  Fig. 4 and  Fig. 5), and (ii) the presence of ATP or ADP prior to open complex formation stimulates NifL inhibition of NifA transcriptional activity in vitro (  Fig. 1).	transcription
60359	5	335582	7	NULL	NULL	0	NULL	ADP	Chemical	presence of	stimulate					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1594_2_243_s_212	11904220	We obtained strong evidence that (i) NifL is able to bind and hydrolyze adenine nucleotides at significant rates (  Fig. 2,  Fig. 3,  Fig. 4 and  Fig. 5), and (ii) the presence of ATP or ADP prior to open complex formation stimulates NifL inhibition of NifA transcriptional activity in vitro (  Fig. 1).	transcription
60360	6	335582	7	NULL	NULL	0	NULL	statement 4	Process		occur prior to					open complex	Process	formation of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1594_2_243_s_212	11904220	We obtained strong evidence that (i) NifL is able to bind and hydrolyze adenine nucleotides at significant rates (  Fig. 2,  Fig. 3,  Fig. 4 and  Fig. 5), and (ii) the presence of ATP or ADP prior to open complex formation stimulates NifL inhibition of NifA transcriptional activity in vitro (  Fig. 1).	transcription
60361	7	335582	7	NULL	NULL	0	NULL	statement 5	Process		occur prior to					open complex	Process	formation of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1594_2_243_s_212	11904220	We obtained strong evidence that (i) NifL is able to bind and hydrolyze adenine nucleotides at significant rates (  Fig. 2,  Fig. 3,  Fig. 4 and  Fig. 5), and (ii) the presence of ATP or ADP prior to open complex formation stimulates NifL inhibition of NifA transcriptional activity in vitro (  Fig. 1).	transcription
60362	8	335582	7	NULL	NULL	0	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1594_2_243_s_212	11904220	We obtained strong evidence that (i) NifL is able to bind and hydrolyze adenine nucleotides at significant rates (  Fig. 2,  Fig. 3,  Fig. 4 and  Fig. 5), and (ii) the presence of ATP or ADP prior to open complex formation stimulates NifL inhibition of NifA transcriptional activity in vitro (  Fig. 1).	transcription
55314	1	335583	5	NULL	NULL	0	NULL	nucleoside transporters			is sensitive to					NBMPR					NULL		0	NULL	NULL	NULL	gw60_circulationres_90_5_570_s_146	11909821	5, 38, 39 Thus, the inhibition of adenosine transport by elevated D-glucose and adenine or uridine nucleotides could be due to the reduced number rather than the activity of an existing pool of NBMPR-sensitive nucleoside transporters in the plasma membrane of HUVECs.	transcription
55315	2	335583	5	NULL	NULL	0	NULL	statement 1			is present in					HUVECs		plasma membrane			NULL		0	NULL	NULL	NULL	gw60_circulationres_90_5_570_s_146	11909821	5, 38, 39 Thus, the inhibition of adenosine transport by elevated D-glucose and adenine or uridine nucleotides could be due to the reduced number rather than the activity of an existing pool of NBMPR-sensitive nucleoside transporters in the plasma membrane of HUVECs.	transcription
55316	3	335583	5	NULL	NULL	0	NULL	D-glucose		elevated 	inhibits					adenosine		transport of			NULL	plasma membrane of HUVECs	NULL	NULL	NULL	NULL	gw60_circulationres_90_5_570_s_146	11909821	5, 38, 39 Thus, the inhibition of adenosine transport by elevated D-glucose and adenine or uridine nucleotides could be due to the reduced number rather than the activity of an existing pool of NBMPR-sensitive nucleoside transporters in the plasma membrane of HUVECs.	transcription
55317	4	335583	5	NULL	NULL	0	NULL	statement 1		reduced number of	leads to					statement 3					NULL	plasma membrane of HUVECs	0	NULL	NULL	NULL	gw60_circulationres_90_5_570_s_146	11909821	5, 38, 39 Thus, the inhibition of adenosine transport by elevated D-glucose and adenine or uridine nucleotides could be due to the reduced number rather than the activity of an existing pool of NBMPR-sensitive nucleoside transporters in the plasma membrane of HUVECs.	transcription
55318	5	335583	5	NULL	NULL	0	NULL	adenine nucleotides		elevated	inhibits					adenosine		transport of			NULL	plasma membrane of HUVECs	0	NULL	NULL	NULL	gw60_circulationres_90_5_570_s_146	11909821	5, 38, 39 Thus, the inhibition of adenosine transport by elevated D-glucose and adenine or uridine nucleotides could be due to the reduced number rather than the activity of an existing pool of NBMPR-sensitive nucleoside transporters in the plasma membrane of HUVECs.	transcription
55319	6	335583	5	NULL	NULL	0	NULL	uridine nucleotides		elevated	inhibits					adenosine		transport of			NULL	plasma membrane of HUVECs	0	NULL	NULL	NULL	gw60_circulationres_90_5_570_s_146	11909821	5, 38, 39 Thus, the inhibition of adenosine transport by elevated D-glucose and adenine or uridine nucleotides could be due to the reduced number rather than the activity of an existing pool of NBMPR-sensitive nucleoside transporters in the plasma membrane of HUVECs.	transcription
55321	7	335583	5	NULL	NULL	0	NULL	statement 5			is an alternative to					statement 6					NULL		0	NULL	NULL	NULL	gw60_circulationres_90_5_570_s_146	11909821	5, 38, 39 Thus, the inhibition of adenosine transport by elevated D-glucose and adenine or uridine nucleotides could be due to the reduced number rather than the activity of an existing pool of NBMPR-sensitive nucleoside transporters in the plasma membrane of HUVECs.	transcription
55323	8	335583	5	NULL	NULL	0	NULL	statement 1		reduced number of	leads to					statement 7					NULL	plasma membrane of HUVECs	0	NULL	NULL	NULL	gw60_circulationres_90_5_570_s_146	11909821	5, 38, 39 Thus, the inhibition of adenosine transport by elevated D-glucose and adenine or uridine nucleotides could be due to the reduced number rather than the activity of an existing pool of NBMPR-sensitive nucleoside transporters in the plasma membrane of HUVECs.	transcription
60363	1	335583	7	NULL	NULL	0	NULL	D-glucose	Chemical	elevated	inhibit					adenosine 	Chemical	transport of			NULL		0	NULL	NULL	NULL	gw60_circulationres_90_5_570_s_146	11909821	5, 38, 39 Thus, the inhibition of adenosine transport by elevated D-glucose and adenine or uridine nucleotides could be due to the reduced number rather than the activity of an existing pool of NBMPR-sensitive nucleoside transporters in the plasma membrane of HUVECs.	transcription
60364	2	335583	7	NULL	NULL	0	NULL	adenine nucleotide	NucleicAcid	elevated	inhibit					adenosine	Chemical	transport of			NULL		NULL	NULL	NULL	NULL	gw60_circulationres_90_5_570_s_146	11909821	5, 38, 39 Thus, the inhibition of adenosine transport by elevated D-glucose and adenine or uridine nucleotides could be due to the reduced number rather than the activity of an existing pool of NBMPR-sensitive nucleoside transporters in the plasma membrane of HUVECs.	transcription
60365	3	335583	7	NULL	NULL	0	NULL	uridine nucleotide	NucleicAcid	elevated	inhibit					adenosine	Chemical	transport of			NULL		0	NULL	NULL	NULL	gw60_circulationres_90_5_570_s_146	11909821	5, 38, 39 Thus, the inhibition of adenosine transport by elevated D-glucose and adenine or uridine nucleotides could be due to the reduced number rather than the activity of an existing pool of NBMPR-sensitive nucleoside transporters in the plasma membrane of HUVECs.	transcription
60366	4	335583	7	NULL	NULL	0	NULL	statement 1	Process		is not due to					NBMPR-sensitive nucleoside transporters	Chemical	activity of			NULL	plasma membrane of HUVECs	NULL	NULL	NULL	NULL	gw60_circulationres_90_5_570_s_146	11909821	5, 38, 39 Thus, the inhibition of adenosine transport by elevated D-glucose and adenine or uridine nucleotides could be due to the reduced number rather than the activity of an existing pool of NBMPR-sensitive nucleoside transporters in the plasma membrane of HUVECs.	transcription
60367	5	335583	7	NULL	NULL	0	NULL	statement 2	Process		is not due to					NBMPR-sensitive nucleoside transporters	Chemical	activity of			NULL	plasma membrane of HUVECs	0	NULL	NULL	NULL	gw60_circulationres_90_5_570_s_146	11909821	5, 38, 39 Thus, the inhibition of adenosine transport by elevated D-glucose and adenine or uridine nucleotides could be due to the reduced number rather than the activity of an existing pool of NBMPR-sensitive nucleoside transporters in the plasma membrane of HUVECs.	transcription
60368	6	335583	7	NULL	NULL	0	NULL	statement 3	Process		is not due to					NBMPR-sensitive nucleoside transporters	Chemical	activity of			NULL	plasma membrane of HUVECs	0	NULL	NULL	NULL	gw60_circulationres_90_5_570_s_146	11909821	5, 38, 39 Thus, the inhibition of adenosine transport by elevated D-glucose and adenine or uridine nucleotides could be due to the reduced number rather than the activity of an existing pool of NBMPR-sensitive nucleoside transporters in the plasma membrane of HUVECs.	transcription
55324	2	335584	5	NULL	NULL	0	NULL	Oct-1			bind			Asn-429		statement 1					NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5453_s_333	10409735	The crystal structure of Oct-1 bound to DNA has shown that critical contact is made between a specific amino acid (Asn-429) of Oct-1 and the adenine nucleotide which base pairs with the second thymine of the Octamer motif (5''-A TTA/TGCAT-3'') ( 19).	transcription
55327	1	335584	5	NULL	NULL	0	NULL	DNA			base pairs with			adenine nucleotide		DNA			thymine of Octamer motif (5''-A TTA/TGCAT-3'')		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_8_5453_s_333	10409735	The crystal structure of Oct-1 bound to DNA has shown that critical contact is made between a specific amino acid (Asn-429) of Oct-1 and the adenine nucleotide which base pairs with the second thymine of the Octamer motif (5''-A TTA/TGCAT-3'') ( 19).	transcription
60369	1	335584	7	NULL	NULL	0	NULL	Oct-1	GP		bind					DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_8_5453_s_333	10409735	The crystal structure of Oct-1 bound to DNA has shown that critical contact is made between a specific amino acid (Asn-429) of Oct-1 and the adenine nucleotide which base pairs with the second thymine of the Octamer motif (5''-A TTA/TGCAT-3'') ( 19).	transcription
60370	2	335584	7	NULL	NULL	0	NULL	Oct-1	GP		contact with			Asn-429		adenine nucleotide	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_8_5453_s_333	10409735	The crystal structure of Oct-1 bound to DNA has shown that critical contact is made between a specific amino acid (Asn-429) of Oct-1 and the adenine nucleotide which base pairs with the second thymine of the Octamer motif (5''-A TTA/TGCAT-3'') ( 19).	transcription
60371	3	335584	7	NULL	NULL	0	NULL	adenine nucleotide	NucleicAcid		base pair with					thymine	NucleicAcid			Octamer motif (5''-A TTA/TGCAT-3'')	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_8_5453_s_333	10409735	The crystal structure of Oct-1 bound to DNA has shown that critical contact is made between a specific amino acid (Asn-429) of Oct-1 and the adenine nucleotide which base pairs with the second thymine of the Octamer motif (5''-A TTA/TGCAT-3'') ( 19).	transcription
55328	1	335585	5	NULL	NULL	0	NULL	Tg			pairs with					adenine					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6111_s_298	12167705	Furthermore, under our conditions  E. coli endonuclease IV did not efficiently cleave Tg paired either with adenine or guanine (Fig.  5, lanes 2 and 13), thereby making it unlikely that a mammalian endonuclease IV-like enzyme is responsible for the residual activity ( 16).	transcription
55330	2	335585	5	NULL	NULL	0	NULL	Tg			pairs with					guanine					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6111_s_298	12167705	Furthermore, under our conditions  E. coli endonuclease IV did not efficiently cleave Tg paired either with adenine or guanine (Fig.  5, lanes 2 and 13), thereby making it unlikely that a mammalian endonuclease IV-like enzyme is responsible for the residual activity ( 16).	transcription
55332	3	335585	5	NULL	NULL	0	NULL	endonuclease IV		E. coli	does not cleave		efficiently			statement 1					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6111_s_298	12167705	Furthermore, under our conditions  E. coli endonuclease IV did not efficiently cleave Tg paired either with adenine or guanine (Fig.  5, lanes 2 and 13), thereby making it unlikely that a mammalian endonuclease IV-like enzyme is responsible for the residual activity ( 16).	transcription
55333	4	335585	5	NULL	NULL	0	NULL	endonuclease IV		E. coli	does not cleave		efficiently			statement 2					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6111_s_298	12167705	Furthermore, under our conditions  E. coli endonuclease IV did not efficiently cleave Tg paired either with adenine or guanine (Fig.  5, lanes 2 and 13), thereby making it unlikely that a mammalian endonuclease IV-like enzyme is responsible for the residual activity ( 16).	transcription
55334	5	335585	5	NULL	NULL	0	NULL	statement 1			is an alternative to					statement 2					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6111_s_298	12167705	Furthermore, under our conditions  E. coli endonuclease IV did not efficiently cleave Tg paired either with adenine or guanine (Fig.  5, lanes 2 and 13), thereby making it unlikely that a mammalian endonuclease IV-like enzyme is responsible for the residual activity ( 16).	transcription
60372	1	335585	7	NULL	NULL	0	NULL	Tg 	Chemical		pair with					adenine	Chemical				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6111_s_298	12167705	Furthermore, under our conditions  E. coli endonuclease IV did not efficiently cleave Tg paired either with adenine or guanine (Fig.  5, lanes 2 and 13), thereby making it unlikely that a mammalian endonuclease IV-like enzyme is responsible for the residual activity ( 16).	transcription
60373	2	335585	7	NULL	NULL	0	NULL	Tg	Chemical		pair with					guanine	Chemical				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6111_s_298	12167705	Furthermore, under our conditions  E. coli endonuclease IV did not efficiently cleave Tg paired either with adenine or guanine (Fig.  5, lanes 2 and 13), thereby making it unlikely that a mammalian endonuclease IV-like enzyme is responsible for the residual activity ( 16).	transcription
60374	3	335585	7	NULL	NULL	0	NULL	endonuclease IV	GP	E.coli	does not cleave		efficiently			statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6111_s_298	12167705	Furthermore, under our conditions  E. coli endonuclease IV did not efficiently cleave Tg paired either with adenine or guanine (Fig.  5, lanes 2 and 13), thereby making it unlikely that a mammalian endonuclease IV-like enzyme is responsible for the residual activity ( 16).	transcription
60375	4	335585	7	NULL	NULL	0	NULL	endonuclease IV	GP	E.coli	does not cleave		efficiently			statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6111_s_298	12167705	Furthermore, under our conditions  E. coli endonuclease IV did not efficiently cleave Tg paired either with adenine or guanine (Fig.  5, lanes 2 and 13), thereby making it unlikely that a mammalian endonuclease IV-like enzyme is responsible for the residual activity ( 16).	transcription
60376	5	335585	7	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6111_s_298	12167705	Furthermore, under our conditions  E. coli endonuclease IV did not efficiently cleave Tg paired either with adenine or guanine (Fig.  5, lanes 2 and 13), thereby making it unlikely that a mammalian endonuclease IV-like enzyme is responsible for the residual activity ( 16).	transcription
60377	6	335585	7	NULL	NULL	0	NULL	endonuclease IV-like enzyme	GP 	mammalian	is not responsible for					residual activity	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6111_s_298	12167705	Furthermore, under our conditions  E. coli endonuclease IV did not efficiently cleave Tg paired either with adenine or guanine (Fig.  5, lanes 2 and 13), thereby making it unlikely that a mammalian endonuclease IV-like enzyme is responsible for the residual activity ( 16).	transcription
60378	7	335585	7	NULL	NULL	0	NULL	statement 3	Process		indicate					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6111_s_298	12167705	Furthermore, under our conditions  E. coli endonuclease IV did not efficiently cleave Tg paired either with adenine or guanine (Fig.  5, lanes 2 and 13), thereby making it unlikely that a mammalian endonuclease IV-like enzyme is responsible for the residual activity ( 16).	transcription
60379	8	335585	7	NULL	NULL	0	NULL	statement 4	Process		indicate					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6111_s_298	12167705	Furthermore, under our conditions  E. coli endonuclease IV did not efficiently cleave Tg paired either with adenine or guanine (Fig.  5, lanes 2 and 13), thereby making it unlikely that a mammalian endonuclease IV-like enzyme is responsible for the residual activity ( 16).	transcription
55335	1	335587	5	NULL	NULL	0	NULL	genomic DNA		Sodalis	methylated at		extensively			adenine residues					NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_15_4517_s_128	11443086	Neither the plasmid nor the chromosomal DNA could be digested with Dam-sensitive restriction enzyme  MboI (Fig.  6, lanes 5), while the same DNAs were cleaved with its isoschizomer  Sau3AI (Fig.  6, lanes 4), indicating that  Sodalis genomic as well as plasmid DNAs are extensively methylated at the adenine residues.	transcription
55336	2	335587	5	NULL	NULL	0	NULL	plasmid DNA		Sodalis	methylated at		extensively			adenine residues					NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_183_15_4517_s_128	11443086	Neither the plasmid nor the chromosomal DNA could be digested with Dam-sensitive restriction enzyme  MboI (Fig.  6, lanes 5), while the same DNAs were cleaved with its isoschizomer  Sau3AI (Fig.  6, lanes 4), indicating that  Sodalis genomic as well as plasmid DNAs are extensively methylated at the adenine residues.	transcription
60380	1	335587	7	NULL	NULL	0	NULL	MboI	GP		does not digest					plasmid DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_15_4517_s_128	11443086	Neither the plasmid nor the chromosomal DNA could be digested with Dam-sensitive restriction enzyme  MboI (Fig.  6, lanes 5), while the same DNAs were cleaved with its isoschizomer  Sau3AI (Fig.  6, lanes 4), indicating that  Sodalis genomic as well as plasmid DNAs are extensively methylated at the adenine residues.	transcription
60381	2	335587	7	NULL	NULL	0	NULL	MboI	GP		does not digest					chromosomal DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_15_4517_s_128	11443086	Neither the plasmid nor the chromosomal DNA could be digested with Dam-sensitive restriction enzyme  MboI (Fig.  6, lanes 5), while the same DNAs were cleaved with its isoschizomer  Sau3AI (Fig.  6, lanes 4), indicating that  Sodalis genomic as well as plasmid DNAs are extensively methylated at the adenine residues.	transcription
60382	3	335587	7	NULL	NULL	0	NULL	MboI	GP		is sensitive to					Dam	GP				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_15_4517_s_128	11443086	Neither the plasmid nor the chromosomal DNA could be digested with Dam-sensitive restriction enzyme  MboI (Fig.  6, lanes 5), while the same DNAs were cleaved with its isoschizomer  Sau3AI (Fig.  6, lanes 4), indicating that  Sodalis genomic as well as plasmid DNAs are extensively methylated at the adenine residues.	transcription
60383	4	335587	7	NULL	NULL	0	NULL	Sau3AI	GP		cleaves					plasmid DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_15_4517_s_128	11443086	Neither the plasmid nor the chromosomal DNA could be digested with Dam-sensitive restriction enzyme  MboI (Fig.  6, lanes 5), while the same DNAs were cleaved with its isoschizomer  Sau3AI (Fig.  6, lanes 4), indicating that  Sodalis genomic as well as plasmid DNAs are extensively methylated at the adenine residues.	transcription
60384	5	335587	7	NULL	NULL	0	NULL	Sau3AI	GP		cleaves					chromosomal DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_15_4517_s_128	11443086	Neither the plasmid nor the chromosomal DNA could be digested with Dam-sensitive restriction enzyme  MboI (Fig.  6, lanes 5), while the same DNAs were cleaved with its isoschizomer  Sau3AI (Fig.  6, lanes 4), indicating that  Sodalis genomic as well as plasmid DNAs are extensively methylated at the adenine residues.	transcription
60385	6	335587	7	NULL	NULL	0	NULL	 genomic DNA	NucleicAcid	Sodalis	is methylated at					adenine residues	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_15_4517_s_128	11443086	Neither the plasmid nor the chromosomal DNA could be digested with Dam-sensitive restriction enzyme  MboI (Fig.  6, lanes 5), while the same DNAs were cleaved with its isoschizomer  Sau3AI (Fig.  6, lanes 4), indicating that  Sodalis genomic as well as plasmid DNAs are extensively methylated at the adenine residues.	transcription
60386	7	335587	7	NULL	NULL	0	NULL	plasmid DNAs	NucleicAcid	Sodalis	is methylated at					adenine residues	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_15_4517_s_128	11443086	Neither the plasmid nor the chromosomal DNA could be digested with Dam-sensitive restriction enzyme  MboI (Fig.  6, lanes 5), while the same DNAs were cleaved with its isoschizomer  Sau3AI (Fig.  6, lanes 4), indicating that  Sodalis genomic as well as plasmid DNAs are extensively methylated at the adenine residues.	transcription
60387	8	335587	7	NULL	NULL	0	NULL	statement 4	Process		indicate					statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_15_4517_s_128	11443086	Neither the plasmid nor the chromosomal DNA could be digested with Dam-sensitive restriction enzyme  MboI (Fig.  6, lanes 5), while the same DNAs were cleaved with its isoschizomer  Sau3AI (Fig.  6, lanes 4), indicating that  Sodalis genomic as well as plasmid DNAs are extensively methylated at the adenine residues.	transcription
60388	9	335587	7	NULL	NULL	0	NULL	statement 5	Process		indicate					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_15_4517_s_128	11443086	Neither the plasmid nor the chromosomal DNA could be digested with Dam-sensitive restriction enzyme  MboI (Fig.  6, lanes 5), while the same DNAs were cleaved with its isoschizomer  Sau3AI (Fig.  6, lanes 4), indicating that  Sodalis genomic as well as plasmid DNAs are extensively methylated at the adenine residues.	transcription
60389	10	335587	7	NULL	NULL	0	NULL	Sau3AI	GP		is an isoschizomer of 					MboI 	GP				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_183_15_4517_s_128	11443086	Neither the plasmid nor the chromosomal DNA could be digested with Dam-sensitive restriction enzyme  MboI (Fig.  6, lanes 5), while the same DNAs were cleaved with its isoschizomer  Sau3AI (Fig.  6, lanes 4), indicating that  Sodalis genomic as well as plasmid DNAs are extensively methylated at the adenine residues.	transcription
55337	1	335588	5	NULL	NULL	0	NULL	ACh			is					acetylcholine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26479_s_12	11994289	Thus, in the pancreatic acinar cell the neurotransmitter acetylcholine (ACh) stimulates the release of Ca2+ from the ER via inositol 1,4,5-trisphosphate (IP3), while the hormone cholecystokinin (CCK) evokes Ca2+ release by a complex interaction between the messengers IP3, cyclic ADP- ribose, and nicotinic acid adenine dinucleotide phosphate (NAADP) ( 5).	transcription
55338	2	335588	5	NULL	NULL	0	NULL	ACh			is a type of					neurotransmitter					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26479_s_12	11994289	Thus, in the pancreatic acinar cell the neurotransmitter acetylcholine (ACh) stimulates the release of Ca2+ from the ER via inositol 1,4,5-trisphosphate (IP3), while the hormone cholecystokinin (CCK) evokes Ca2+ release by a complex interaction between the messengers IP3, cyclic ADP- ribose, and nicotinic acid adenine dinucleotide phosphate (NAADP) ( 5).	transcription
55339	3	335588	5	NULL	NULL	0	NULL	Ca2+			is relased from					ER					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26479_s_12	11994289	Thus, in the pancreatic acinar cell the neurotransmitter acetylcholine (ACh) stimulates the release of Ca2+ from the ER via inositol 1,4,5-trisphosphate (IP3), while the hormone cholecystokinin (CCK) evokes Ca2+ release by a complex interaction between the messengers IP3, cyclic ADP- ribose, and nicotinic acid adenine dinucleotide phosphate (NAADP) ( 5).	transcription
55340	4	335588	5	NULL	NULL	0	NULL	statement 3			via					IP3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26479_s_12	11994289	Thus, in the pancreatic acinar cell the neurotransmitter acetylcholine (ACh) stimulates the release of Ca2+ from the ER via inositol 1,4,5-trisphosphate (IP3), while the hormone cholecystokinin (CCK) evokes Ca2+ release by a complex interaction between the messengers IP3, cyclic ADP- ribose, and nicotinic acid adenine dinucleotide phosphate (NAADP) ( 5).	transcription
55341	5	335588	5	NULL	NULL	0	NULL	ACh			stimulates					statement 3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26479_s_12	11994289	Thus, in the pancreatic acinar cell the neurotransmitter acetylcholine (ACh) stimulates the release of Ca2+ from the ER via inositol 1,4,5-trisphosphate (IP3), while the hormone cholecystokinin (CCK) evokes Ca2+ release by a complex interaction between the messengers IP3, cyclic ADP- ribose, and nicotinic acid adenine dinucleotide phosphate (NAADP) ( 5).	transcription
55342	6	335588	5	NULL	NULL	0	NULL	IP3			is					inositol 1,4,5-trisphosphate					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26479_s_12	11994289	Thus, in the pancreatic acinar cell the neurotransmitter acetylcholine (ACh) stimulates the release of Ca2+ from the ER via inositol 1,4,5-trisphosphate (IP3), while the hormone cholecystokinin (CCK) evokes Ca2+ release by a complex interaction between the messengers IP3, cyclic ADP- ribose, and nicotinic acid adenine dinucleotide phosphate (NAADP) ( 5).	transcription
55343	7	335588	5	NULL	NULL	0	NULL	CCK			is					cholecystokinin					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26479_s_12	11994289	Thus, in the pancreatic acinar cell the neurotransmitter acetylcholine (ACh) stimulates the release of Ca2+ from the ER via inositol 1,4,5-trisphosphate (IP3), while the hormone cholecystokinin (CCK) evokes Ca2+ release by a complex interaction between the messengers IP3, cyclic ADP- ribose, and nicotinic acid adenine dinucleotide phosphate (NAADP) ( 5).	transcription
55344	8	335588	5	NULL	NULL	0	NULL	CCK			is a type of					hormone					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26479_s_12	11994289	Thus, in the pancreatic acinar cell the neurotransmitter acetylcholine (ACh) stimulates the release of Ca2+ from the ER via inositol 1,4,5-trisphosphate (IP3), while the hormone cholecystokinin (CCK) evokes Ca2+ release by a complex interaction between the messengers IP3, cyclic ADP- ribose, and nicotinic acid adenine dinucleotide phosphate (NAADP) ( 5).	transcription
55345	9	335588	5	NULL	NULL	0	NULL	IP3			is a type of					messenger					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26479_s_12	11994289	Thus, in the pancreatic acinar cell the neurotransmitter acetylcholine (ACh) stimulates the release of Ca2+ from the ER via inositol 1,4,5-trisphosphate (IP3), while the hormone cholecystokinin (CCK) evokes Ca2+ release by a complex interaction between the messengers IP3, cyclic ADP- ribose, and nicotinic acid adenine dinucleotide phosphate (NAADP) ( 5).	transcription
55346	10	335588	5	NULL	NULL	0	NULL	cyclic ADP- ribose			is a type of					messenger					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26479_s_12	11994289	Thus, in the pancreatic acinar cell the neurotransmitter acetylcholine (ACh) stimulates the release of Ca2+ from the ER via inositol 1,4,5-trisphosphate (IP3), while the hormone cholecystokinin (CCK) evokes Ca2+ release by a complex interaction between the messengers IP3, cyclic ADP- ribose, and nicotinic acid adenine dinucleotide phosphate (NAADP) ( 5).	transcription
55348	11	335588	5	NULL	NULL	0	NULL	NAADP			is a type of					messenger					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26479_s_12	11994289	Thus, in the pancreatic acinar cell the neurotransmitter acetylcholine (ACh) stimulates the release of Ca2+ from the ER via inositol 1,4,5-trisphosphate (IP3), while the hormone cholecystokinin (CCK) evokes Ca2+ release by a complex interaction between the messengers IP3, cyclic ADP- ribose, and nicotinic acid adenine dinucleotide phosphate (NAADP) ( 5).	transcription
55349	12	335588	5	NULL	NULL	0	NULL	NAADP			is					nicotinic acid adenine dinucleotide phosphate					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26479_s_12	11994289	Thus, in the pancreatic acinar cell the neurotransmitter acetylcholine (ACh) stimulates the release of Ca2+ from the ER via inositol 1,4,5-trisphosphate (IP3), while the hormone cholecystokinin (CCK) evokes Ca2+ release by a complex interaction between the messengers IP3, cyclic ADP- ribose, and nicotinic acid adenine dinucleotide phosphate (NAADP) ( 5).	transcription
55350	13	335588	5	NULL	NULL	0	NULL	IP3			interacts with					cyclic ADP- ribose					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26479_s_12	11994289	Thus, in the pancreatic acinar cell the neurotransmitter acetylcholine (ACh) stimulates the release of Ca2+ from the ER via inositol 1,4,5-trisphosphate (IP3), while the hormone cholecystokinin (CCK) evokes Ca2+ release by a complex interaction between the messengers IP3, cyclic ADP- ribose, and nicotinic acid adenine dinucleotide phosphate (NAADP) ( 5).	transcription
55351	14	335588	5	NULL	NULL	0	NULL	IP3			interacts with					NAADP					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26479_s_12	11994289	Thus, in the pancreatic acinar cell the neurotransmitter acetylcholine (ACh) stimulates the release of Ca2+ from the ER via inositol 1,4,5-trisphosphate (IP3), while the hormone cholecystokinin (CCK) evokes Ca2+ release by a complex interaction between the messengers IP3, cyclic ADP- ribose, and nicotinic acid adenine dinucleotide phosphate (NAADP) ( 5).	transcription
55352	15	335588	5	NULL	NULL	0	NULL	statement 13			occurs simultaneously with					statement 14					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26479_s_12	11994289	Thus, in the pancreatic acinar cell the neurotransmitter acetylcholine (ACh) stimulates the release of Ca2+ from the ER via inositol 1,4,5-trisphosphate (IP3), while the hormone cholecystokinin (CCK) evokes Ca2+ release by a complex interaction between the messengers IP3, cyclic ADP- ribose, and nicotinic acid adenine dinucleotide phosphate (NAADP) ( 5).	transcription
55353	16	335588	5	NULL	NULL	0	NULL	Ca2+			is released by					statement 15					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26479_s_12	11994289	Thus, in the pancreatic acinar cell the neurotransmitter acetylcholine (ACh) stimulates the release of Ca2+ from the ER via inositol 1,4,5-trisphosphate (IP3), while the hormone cholecystokinin (CCK) evokes Ca2+ release by a complex interaction between the messengers IP3, cyclic ADP- ribose, and nicotinic acid adenine dinucleotide phosphate (NAADP) ( 5).	transcription
55354	17	335588	5	NULL	NULL	0	NULL	CCK			evokes					statement 16					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26479_s_12	11994289	Thus, in the pancreatic acinar cell the neurotransmitter acetylcholine (ACh) stimulates the release of Ca2+ from the ER via inositol 1,4,5-trisphosphate (IP3), while the hormone cholecystokinin (CCK) evokes Ca2+ release by a complex interaction between the messengers IP3, cyclic ADP- ribose, and nicotinic acid adenine dinucleotide phosphate (NAADP) ( 5).	transcription
60390	1	335588	7	NULL	NULL	0	NULL	ACh	Chemical		stimulates					Ca2+	Chemical	release of			NULL	pancreatic acinar cell 	0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26479_s_12	11994289	Thus, in the pancreatic acinar cell the neurotransmitter acetylcholine (ACh) stimulates the release of Ca2+ from the ER via inositol 1,4,5-trisphosphate (IP3), while the hormone cholecystokinin (CCK) evokes Ca2+ release by a complex interaction between the messengers IP3, cyclic ADP- ribose, and nicotinic acid adenine dinucleotide phosphate (NAADP) ( 5).	transcription
60391	2	335588	7	NULL	NULL	0	NULL	statement 1	Process		occur from					ER	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26479_s_12	11994289	Thus, in the pancreatic acinar cell the neurotransmitter acetylcholine (ACh) stimulates the release of Ca2+ from the ER via inositol 1,4,5-trisphosphate (IP3), while the hormone cholecystokinin (CCK) evokes Ca2+ release by a complex interaction between the messengers IP3, cyclic ADP- ribose, and nicotinic acid adenine dinucleotide phosphate (NAADP) ( 5).	transcription
60392	3	335588	7	NULL	NULL	0	NULL	statement 2	Process		occur via					IP3	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26479_s_12	11994289	Thus, in the pancreatic acinar cell the neurotransmitter acetylcholine (ACh) stimulates the release of Ca2+ from the ER via inositol 1,4,5-trisphosphate (IP3), while the hormone cholecystokinin (CCK) evokes Ca2+ release by a complex interaction between the messengers IP3, cyclic ADP- ribose, and nicotinic acid adenine dinucleotide phosphate (NAADP) ( 5).	transcription
60393	4	335588	7	NULL	NULL	0	NULL	CCK	GP		evokes					Ca2+	Chemical	release of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26479_s_12	11994289	Thus, in the pancreatic acinar cell the neurotransmitter acetylcholine (ACh) stimulates the release of Ca2+ from the ER via inositol 1,4,5-trisphosphate (IP3), while the hormone cholecystokinin (CCK) evokes Ca2+ release by a complex interaction between the messengers IP3, cyclic ADP- ribose, and nicotinic acid adenine dinucleotide phosphate (NAADP) ( 5).	transcription
60394	5	335588	7	NULL	NULL	0	NULL	IP3	Chemical		interacts with					cyclic ADP- ribose	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26479_s_12	11994289	Thus, in the pancreatic acinar cell the neurotransmitter acetylcholine (ACh) stimulates the release of Ca2+ from the ER via inositol 1,4,5-trisphosphate (IP3), while the hormone cholecystokinin (CCK) evokes Ca2+ release by a complex interaction between the messengers IP3, cyclic ADP- ribose, and nicotinic acid adenine dinucleotide phosphate (NAADP) ( 5).	transcription
60395	6	335588	7	NULL	NULL	0	NULL	statement 5	Process		interacts with					NAADP	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26479_s_12	11994289	Thus, in the pancreatic acinar cell the neurotransmitter acetylcholine (ACh) stimulates the release of Ca2+ from the ER via inositol 1,4,5-trisphosphate (IP3), while the hormone cholecystokinin (CCK) evokes Ca2+ release by a complex interaction between the messengers IP3, cyclic ADP- ribose, and nicotinic acid adenine dinucleotide phosphate (NAADP) ( 5).	transcription
60396	7	335588	7	NULL	NULL	0	NULL	statement 4	Process		occur by					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26479_s_12	11994289	Thus, in the pancreatic acinar cell the neurotransmitter acetylcholine (ACh) stimulates the release of Ca2+ from the ER via inositol 1,4,5-trisphosphate (IP3), while the hormone cholecystokinin (CCK) evokes Ca2+ release by a complex interaction between the messengers IP3, cyclic ADP- ribose, and nicotinic acid adenine dinucleotide phosphate (NAADP) ( 5).	transcription
60397	8	335588	7	NULL	NULL	0	NULL	statement 4	Process		occur by					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26479_s_12	11994289	Thus, in the pancreatic acinar cell the neurotransmitter acetylcholine (ACh) stimulates the release of Ca2+ from the ER via inositol 1,4,5-trisphosphate (IP3), while the hormone cholecystokinin (CCK) evokes Ca2+ release by a complex interaction between the messengers IP3, cyclic ADP- ribose, and nicotinic acid adenine dinucleotide phosphate (NAADP) ( 5).	transcription
60398	9	335588	7	NULL	NULL	0	NULL	ACh	Chemical		is a type of					neurotransmitter	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26479_s_12	11994289	Thus, in the pancreatic acinar cell the neurotransmitter acetylcholine (ACh) stimulates the release of Ca2+ from the ER via inositol 1,4,5-trisphosphate (IP3), while the hormone cholecystokinin (CCK) evokes Ca2+ release by a complex interaction between the messengers IP3, cyclic ADP- ribose, and nicotinic acid adenine dinucleotide phosphate (NAADP) ( 5).	transcription
60399	10	335588	7	NULL	NULL	0	NULL	ACh	Chemical		is					acetylcholine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26479_s_12	11994289	Thus, in the pancreatic acinar cell the neurotransmitter acetylcholine (ACh) stimulates the release of Ca2+ from the ER via inositol 1,4,5-trisphosphate (IP3), while the hormone cholecystokinin (CCK) evokes Ca2+ release by a complex interaction between the messengers IP3, cyclic ADP- ribose, and nicotinic acid adenine dinucleotide phosphate (NAADP) ( 5).	transcription
60400	11	335588	7	NULL	NULL	0	NULL	IP3	Chemical		is					inositol 1,4,5-trisphosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26479_s_12	11994289	Thus, in the pancreatic acinar cell the neurotransmitter acetylcholine (ACh) stimulates the release of Ca2+ from the ER via inositol 1,4,5-trisphosphate (IP3), while the hormone cholecystokinin (CCK) evokes Ca2+ release by a complex interaction between the messengers IP3, cyclic ADP- ribose, and nicotinic acid adenine dinucleotide phosphate (NAADP) ( 5).	transcription
60401	12	335588	7	NULL	NULL	0	NULL	CCK	GP		is					cholecystokinin	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26479_s_12	11994289	Thus, in the pancreatic acinar cell the neurotransmitter acetylcholine (ACh) stimulates the release of Ca2+ from the ER via inositol 1,4,5-trisphosphate (IP3), while the hormone cholecystokinin (CCK) evokes Ca2+ release by a complex interaction between the messengers IP3, cyclic ADP- ribose, and nicotinic acid adenine dinucleotide phosphate (NAADP) ( 5).	transcription
60402	13	335588	7	NULL	NULL	0	NULL	NAADP	Chemical		is					nicotinic acid adenine dinucleotide phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_26479_s_12	11994289	Thus, in the pancreatic acinar cell the neurotransmitter acetylcholine (ACh) stimulates the release of Ca2+ from the ER via inositol 1,4,5-trisphosphate (IP3), while the hormone cholecystokinin (CCK) evokes Ca2+ release by a complex interaction between the messengers IP3, cyclic ADP- ribose, and nicotinic acid adenine dinucleotide phosphate (NAADP) ( 5).	transcription
55358	1	335589	5	NULL	NULL	0	NULL	succinate dehydrogenase			is activated by					adenine nucleotides					NULL	cauliflower mitochondria	0	NULL	NULL	NULL	gw60_jbiolchem_276_35_32567_s_233	11350973	This observation agrees well with the earlier findings that activation of succinate dehydrogenase by adenine nucleotides in cauliflower mitochondria is negatively affected by sonication or freeze-thawing treatments ( 5) and that the mammalian succinate dehydrogenase is not at all activated by ATP when studied in a solubilized form or in sub-mitochondrial particles ( 3).	transcription
55360	2	335589	5	NULL	NULL	0	NULL	sonication		treatment	affects		negatively			statement 1					NULL	cauliflower mitochondria	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_35_32567_s_233	11350973	This observation agrees well with the earlier findings that activation of succinate dehydrogenase by adenine nucleotides in cauliflower mitochondria is negatively affected by sonication or freeze-thawing treatments ( 5) and that the mammalian succinate dehydrogenase is not at all activated by ATP when studied in a solubilized form or in sub-mitochondrial particles ( 3).	transcription
55361	3	335589	5	NULL	NULL	0	NULL	freeze-thawing		treatment	affects		negatively			statement 1					NULL	cauliflower mitochondria	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_35_32567_s_233	11350973	This observation agrees well with the earlier findings that activation of succinate dehydrogenase by adenine nucleotides in cauliflower mitochondria is negatively affected by sonication or freeze-thawing treatments ( 5) and that the mammalian succinate dehydrogenase is not at all activated by ATP when studied in a solubilized form or in sub-mitochondrial particles ( 3).	transcription
55362	4	335589	5	NULL	NULL	0	NULL	statement 2			is an alternative to					statement 3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_35_32567_s_233	11350973	This observation agrees well with the earlier findings that activation of succinate dehydrogenase by adenine nucleotides in cauliflower mitochondria is negatively affected by sonication or freeze-thawing treatments ( 5) and that the mammalian succinate dehydrogenase is not at all activated by ATP when studied in a solubilized form or in sub-mitochondrial particles ( 3).	transcription
55364	5	335589	5	NULL	NULL	0	NULL	succinate dehydrogenase		mammalian;;soluble	is not activated by					ATP					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_35_32567_s_233	11350973	This observation agrees well with the earlier findings that activation of succinate dehydrogenase by adenine nucleotides in cauliflower mitochondria is negatively affected by sonication or freeze-thawing treatments ( 5) and that the mammalian succinate dehydrogenase is not at all activated by ATP when studied in a solubilized form or in sub-mitochondrial particles ( 3).	transcription
55366	6	335589	5	NULL	NULL	0	NULL	succinate dehydrogenase		mammalian	is not activated by					ATP					NULL	sub-mitochondrial particles	0	NULL	NULL	NULL	gw60_jbiolchem_276_35_32567_s_233	11350973	This observation agrees well with the earlier findings that activation of succinate dehydrogenase by adenine nucleotides in cauliflower mitochondria is negatively affected by sonication or freeze-thawing treatments ( 5) and that the mammalian succinate dehydrogenase is not at all activated by ATP when studied in a solubilized form or in sub-mitochondrial particles ( 3).	transcription
60403	1	335589	7	NULL	NULL	0	NULL	adenine nucleotides	NucleicAcid		activates					succinate dehydrogenase	GP				NULL	cauliflower mitochondria	0	NULL	NULL	NULL	gw60_jbiolchem_276_35_32567_s_233	11350973	This observation agrees well with the earlier findings that activation of succinate dehydrogenase by adenine nucleotides in cauliflower mitochondria is negatively affected by sonication or freeze-thawing treatments ( 5) and that the mammalian succinate dehydrogenase is not at all activated by ATP when studied in a solubilized form or in sub-mitochondrial particles ( 3).	transcription
60404	2	335589	7	NULL	NULL	0	NULL	statement 1	Process		affected by		negatively			sonication	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_35_32567_s_233	11350973	This observation agrees well with the earlier findings that activation of succinate dehydrogenase by adenine nucleotides in cauliflower mitochondria is negatively affected by sonication or freeze-thawing treatments ( 5) and that the mammalian succinate dehydrogenase is not at all activated by ATP when studied in a solubilized form or in sub-mitochondrial particles ( 3).	transcription
60405	3	335589	7	NULL	NULL	0	NULL	statement 1	Process		affected by		negatively			freeze-thawing	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_35_32567_s_233	11350973	This observation agrees well with the earlier findings that activation of succinate dehydrogenase by adenine nucleotides in cauliflower mitochondria is negatively affected by sonication or freeze-thawing treatments ( 5) and that the mammalian succinate dehydrogenase is not at all activated by ATP when studied in a solubilized form or in sub-mitochondrial particles ( 3).	transcription
60406	4	335589	7	NULL	NULL	0	NULL	 ATP	Chemical		does not activate					succinate dehydrogenase	GP	mammalian			NULL	sub-mitochondrial particles 	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_35_32567_s_233	11350973	This observation agrees well with the earlier findings that activation of succinate dehydrogenase by adenine nucleotides in cauliflower mitochondria is negatively affected by sonication or freeze-thawing treatments ( 5) and that the mammalian succinate dehydrogenase is not at all activated by ATP when studied in a solubilized form or in sub-mitochondrial particles ( 3).	transcription
60407	5	335589	7	NULL	NULL	0	NULL	ATP	Chemical		does not activate					succinate dehydrogenase	GP	mammalian;;solubilized			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_35_32567_s_233	11350973	This observation agrees well with the earlier findings that activation of succinate dehydrogenase by adenine nucleotides in cauliflower mitochondria is negatively affected by sonication or freeze-thawing treatments ( 5) and that the mammalian succinate dehydrogenase is not at all activated by ATP when studied in a solubilized form or in sub-mitochondrial particles ( 3).	transcription
55368	1	335590	5	NULL	NULL	0	NULL	oligonucleotide duplex		synthetic	carries									abasic site	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_25_15650_s_165	9188454	A recent methylation interference analysis of Ape interaction with a synthetic oligonucleotide duplex carrying an abasic site on one strand displayed a substantial interference signal from an adenine two nucleotides 5  to the abasic site (equivalent to the guanine lying between the two thymines marked in Fig.  7) ( 35).	transcription
55369	2	335590	5	NULL	NULL	0	NULL	Ape			interacts with					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_25_15650_s_165	9188454	A recent methylation interference analysis of Ape interaction with a synthetic oligonucleotide duplex carrying an abasic site on one strand displayed a substantial interference signal from an adenine two nucleotides 5  to the abasic site (equivalent to the guanine lying between the two thymines marked in Fig.  7) ( 35).	transcription
60408	1	335590	7	NULL	NULL	0	NULL	oligonucleotide duplex 	NucleicAcid		carry									abasic site on one strand 	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_25_15650_s_165	9188454	A recent methylation interference analysis of Ape interaction with a synthetic oligonucleotide duplex carrying an abasic site on one strand displayed a substantial interference signal from an adenine two nucleotides 5  to the abasic site (equivalent to the guanine lying between the two thymines marked in Fig.  7) ( 35).	transcription
60409	2	335590	7	NULL	NULL	0	NULL	Ape	Chemical		interacts with					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_25_15650_s_165	9188454	A recent methylation interference analysis of Ape interaction with a synthetic oligonucleotide duplex carrying an abasic site on one strand displayed a substantial interference signal from an adenine two nucleotides 5  to the abasic site (equivalent to the guanine lying between the two thymines marked in Fig.  7) ( 35).	transcription
60410	3	335590	7	NULL	NULL	0	NULL	statement 2	Process		is interferred by					adenine	Chemical	signal from			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_25_15650_s_165	9188454	A recent methylation interference analysis of Ape interaction with a synthetic oligonucleotide duplex carrying an abasic site on one strand displayed a substantial interference signal from an adenine two nucleotides 5  to the abasic site (equivalent to the guanine lying between the two thymines marked in Fig.  7) ( 35).	transcription
60411	4	335590	7	NULL	NULL	0	NULL	adenine	Chemical		is located at									two nucleotides 5 to the abasic site	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_25_15650_s_165	9188454	A recent methylation interference analysis of Ape interaction with a synthetic oligonucleotide duplex carrying an abasic site on one strand displayed a substantial interference signal from an adenine two nucleotides 5  to the abasic site (equivalent to the guanine lying between the two thymines marked in Fig.  7) ( 35).	transcription
55383	1	335591	5	NULL	NULL	0	NULL	ScCKmit			couple with		functionally			ATP-ADP carrier					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_10_6937_s_24	10702255	Considering the functional coupling of the ScCKmit with the ATP-ADP carrier and the restricted permeability of the outer mitochondrial membrane for adenine nucleotides ( 5,  14), the ADP produced in the intermembrane space by ScCKmit could be more efficient to stimulate the respiration than ADP produced directly in the cytoplasm ( 15).	transcription
55384	2	335591	5	NULL	NULL	0	NULL	mitochondrial membrane		outer	permiable to		restricted			adenine nucleotides					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_10_6937_s_24	10702255	Considering the functional coupling of the ScCKmit with the ATP-ADP carrier and the restricted permeability of the outer mitochondrial membrane for adenine nucleotides ( 5,  14), the ADP produced in the intermembrane space by ScCKmit could be more efficient to stimulate the respiration than ADP produced directly in the cytoplasm ( 15).	transcription
55385	3	335591	5	NULL	NULL	0	NULL	ADP			is produced by					ScCKmit					NULL	intermembrane space	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_10_6937_s_24	10702255	Considering the functional coupling of the ScCKmit with the ATP-ADP carrier and the restricted permeability of the outer mitochondrial membrane for adenine nucleotides ( 5,  14), the ADP produced in the intermembrane space by ScCKmit could be more efficient to stimulate the respiration than ADP produced directly in the cytoplasm ( 15).	transcription
55387	4	335591	5	NULL	NULL	0	NULL	ADP			is produced in		directly			cytoplasm					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_10_6937_s_24	10702255	Considering the functional coupling of the ScCKmit with the ATP-ADP carrier and the restricted permeability of the outer mitochondrial membrane for adenine nucleotides ( 5,  14), the ADP produced in the intermembrane space by ScCKmit could be more efficient to stimulate the respiration than ADP produced directly in the cytoplasm ( 15).	transcription
55391	5	335591	5	NULL	NULL	0	NULL	statement 3			stimulates					respiration					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_10_6937_s_24	10702255	Considering the functional coupling of the ScCKmit with the ATP-ADP carrier and the restricted permeability of the outer mitochondrial membrane for adenine nucleotides ( 5,  14), the ADP produced in the intermembrane space by ScCKmit could be more efficient to stimulate the respiration than ADP produced directly in the cytoplasm ( 15).	transcription
55392	6	335591	5	NULL	NULL	0	NULL	statement 4			stimulates					respiration					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_10_6937_s_24	10702255	Considering the functional coupling of the ScCKmit with the ATP-ADP carrier and the restricted permeability of the outer mitochondrial membrane for adenine nucleotides ( 5,  14), the ADP produced in the intermembrane space by ScCKmit could be more efficient to stimulate the respiration than ADP produced directly in the cytoplasm ( 15).	transcription
55393	7	335591	5	NULL	NULL	0	NULL	statement 5			more efficient than					statement 8					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_10_6937_s_24	10702255	Considering the functional coupling of the ScCKmit with the ATP-ADP carrier and the restricted permeability of the outer mitochondrial membrane for adenine nucleotides ( 5,  14), the ADP produced in the intermembrane space by ScCKmit could be more efficient to stimulate the respiration than ADP produced directly in the cytoplasm ( 15).	transcription
60412	1	335591	7	NULL	NULL	0	NULL	ScCKmit	GP		coupled with		functionally			ATP-ADP carrier	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_10_6937_s_24	10702255	Considering the functional coupling of the ScCKmit with the ATP-ADP carrier and the restricted permeability of the outer mitochondrial membrane for adenine nucleotides ( 5,  14), the ADP produced in the intermembrane space by ScCKmit could be more efficient to stimulate the respiration than ADP produced directly in the cytoplasm ( 15).	transcription
60413	2	335591	7	NULL	NULL	0	NULL	adenine nucleotides	Chemical	permeability of	restricted to					outer mitochondrial membrane	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_10_6937_s_24	10702255	Considering the functional coupling of the ScCKmit with the ATP-ADP carrier and the restricted permeability of the outer mitochondrial membrane for adenine nucleotides ( 5,  14), the ADP produced in the intermembrane space by ScCKmit could be more efficient to stimulate the respiration than ADP produced directly in the cytoplasm ( 15).	transcription
60414	3	335591	7	NULL	NULL	0	NULL	 ScCKmit	GP		produce					ADP	Chemical				NULL	 intermembrane space	0	NULL	NULL	NULL	gw60_jbiolchem_275_10_6937_s_24	10702255	Considering the functional coupling of the ScCKmit with the ATP-ADP carrier and the restricted permeability of the outer mitochondrial membrane for adenine nucleotides ( 5,  14), the ADP produced in the intermembrane space by ScCKmit could be more efficient to stimulate the respiration than ADP produced directly in the cytoplasm ( 15).	transcription
60415	4	335591	7	NULL	NULL	0	NULL	statement 3	Process		stimulate					respiration	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_10_6937_s_24	10702255	Considering the functional coupling of the ScCKmit with the ATP-ADP carrier and the restricted permeability of the outer mitochondrial membrane for adenine nucleotides ( 5,  14), the ADP produced in the intermembrane space by ScCKmit could be more efficient to stimulate the respiration than ADP produced directly in the cytoplasm ( 15).	transcription
60416	5	335591	7	NULL	NULL	0	NULL	ADP	Chemical		produced in		directly			cytoplasm	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_10_6937_s_24	10702255	Considering the functional coupling of the ScCKmit with the ATP-ADP carrier and the restricted permeability of the outer mitochondrial membrane for adenine nucleotides ( 5,  14), the ADP produced in the intermembrane space by ScCKmit could be more efficient to stimulate the respiration than ADP produced directly in the cytoplasm ( 15).	transcription
60417	6	335591	7	NULL	NULL	0	NULL	statement 5	Process		stimulate					respiration	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_10_6937_s_24	10702255	Considering the functional coupling of the ScCKmit with the ATP-ADP carrier and the restricted permeability of the outer mitochondrial membrane for adenine nucleotides ( 5,  14), the ADP produced in the intermembrane space by ScCKmit could be more efficient to stimulate the respiration than ADP produced directly in the cytoplasm ( 15).	transcription
60418	7	335591	7	NULL	NULL	0	NULL	statement 4	Process		is more efficient than					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_10_6937_s_24	10702255	Considering the functional coupling of the ScCKmit with the ATP-ADP carrier and the restricted permeability of the outer mitochondrial membrane for adenine nucleotides ( 5,  14), the ADP produced in the intermembrane space by ScCKmit could be more efficient to stimulate the respiration than ADP produced directly in the cytoplasm ( 15).	transcription
55394	1	335592	5	NULL	NULL	0	NULL	adenine nucleotide			promotes					Cl channel activation					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_46_29080_s_7	8910562	Although injection of oocytes with either GDPbetaS (guanyl-5 -yl thiophosphate) or GTPgammaS (guanosine 5 -3- O-(thio)triphosphate) resulted in loss of adenine nucleotide-promoted Cl  channel activation, neither guanine nucleotide altered the 2MeSATP-stimulated cation current.	transcription
55395	2	335592	5	NULL	NULL	0	NULL	oocytes			is injected with					GDPbetaS (guanyl-5 -yl thiophosphate)					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_46_29080_s_7	8910562	Although injection of oocytes with either GDPbetaS (guanyl-5 -yl thiophosphate) or GTPgammaS (guanosine 5 -3- O-(thio)triphosphate) resulted in loss of adenine nucleotide-promoted Cl  channel activation, neither guanine nucleotide altered the 2MeSATP-stimulated cation current.	transcription
55397	3	335592	5	NULL	NULL	0	NULL	oocytes			is injected with					GTPgammaS (guanosine 5 -3- O-(thio)triphosphate)					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_46_29080_s_7	8910562	Although injection of oocytes with either GDPbetaS (guanyl-5 -yl thiophosphate) or GTPgammaS (guanosine 5 -3- O-(thio)triphosphate) resulted in loss of adenine nucleotide-promoted Cl  channel activation, neither guanine nucleotide altered the 2MeSATP-stimulated cation current.	transcription
55398	4	335592	5	NULL	NULL	0	NULL	statement 2			is an alternative to					statement 3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_46_29080_s_7	8910562	Although injection of oocytes with either GDPbetaS (guanyl-5 -yl thiophosphate) or GTPgammaS (guanosine 5 -3- O-(thio)triphosphate) resulted in loss of adenine nucleotide-promoted Cl  channel activation, neither guanine nucleotide altered the 2MeSATP-stimulated cation current.	transcription
55404	5	335592	5	NULL	NULL	0	NULL	statement 2			results in					statement 1		loss of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_46_29080_s_7	8910562	Although injection of oocytes with either GDPbetaS (guanyl-5 -yl thiophosphate) or GTPgammaS (guanosine 5 -3- O-(thio)triphosphate) resulted in loss of adenine nucleotide-promoted Cl  channel activation, neither guanine nucleotide altered the 2MeSATP-stimulated cation current.	transcription
55405	6	335592	5	NULL	NULL	0	NULL	statement 3			results in					statement 1		loss of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_46_29080_s_7	8910562	Although injection of oocytes with either GDPbetaS (guanyl-5 -yl thiophosphate) or GTPgammaS (guanosine 5 -3- O-(thio)triphosphate) resulted in loss of adenine nucleotide-promoted Cl  channel activation, neither guanine nucleotide altered the 2MeSATP-stimulated cation current.	transcription
55406	7	335592	5	NULL	NULL	0	NULL	2MeSATP			stimulates					cation current					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_46_29080_s_7	8910562	Although injection of oocytes with either GDPbetaS (guanyl-5 -yl thiophosphate) or GTPgammaS (guanosine 5 -3- O-(thio)triphosphate) resulted in loss of adenine nucleotide-promoted Cl  channel activation, neither guanine nucleotide altered the 2MeSATP-stimulated cation current.	transcription
55407	8	335592	5	NULL	NULL	0	NULL	GDPbetaS (guanyl-5 -yl thiophosphate)			does not alter					statement 7					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_46_29080_s_7	8910562	Although injection of oocytes with either GDPbetaS (guanyl-5 -yl thiophosphate) or GTPgammaS (guanosine 5 -3- O-(thio)triphosphate) resulted in loss of adenine nucleotide-promoted Cl  channel activation, neither guanine nucleotide altered the 2MeSATP-stimulated cation current.	transcription
55408	9	335592	5	NULL	NULL	0	NULL	GTPgammaS (guanosine 5 -3- O-(thio)triphosphate)			does not alter					statement 7					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_46_29080_s_7	8910562	Although injection of oocytes with either GDPbetaS (guanyl-5 -yl thiophosphate) or GTPgammaS (guanosine 5 -3- O-(thio)triphosphate) resulted in loss of adenine nucleotide-promoted Cl  channel activation, neither guanine nucleotide altered the 2MeSATP-stimulated cation current.	transcription
60419	1	335592	7	NULL	NULL	0	NULL	adenine nucleotide	NucleicAcid		promote					Cl channel	CellComponent	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_46_29080_s_7	8910562	Although injection of oocytes with either GDPbetaS (guanyl-5 -yl thiophosphate) or GTPgammaS (guanosine 5 -3- O-(thio)triphosphate) resulted in loss of adenine nucleotide-promoted Cl  channel activation, neither guanine nucleotide altered the 2MeSATP-stimulated cation current.	transcription
60420	2	335592	7	NULL	NULL	0	NULL	GDPbetaS (guanyl-5 -yl thiophosphate)	Chemical	treatment with	results in					statement 1	Process	loss of			NULL	oocytes	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_46_29080_s_7	8910562	Although injection of oocytes with either GDPbetaS (guanyl-5 -yl thiophosphate) or GTPgammaS (guanosine 5 -3- O-(thio)triphosphate) resulted in loss of adenine nucleotide-promoted Cl  channel activation, neither guanine nucleotide altered the 2MeSATP-stimulated cation current.	transcription
60421	3	335592	7	NULL	NULL	0	NULL	GTPgammaS (guanosine 5 -3- O-(thio)triphosphate)	Chemical	treatment with	results in					statement 1	Process	loss of			NULL	oocytes	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_46_29080_s_7	8910562	Although injection of oocytes with either GDPbetaS (guanyl-5 -yl thiophosphate) or GTPgammaS (guanosine 5 -3- O-(thio)triphosphate) resulted in loss of adenine nucleotide-promoted Cl  channel activation, neither guanine nucleotide altered the 2MeSATP-stimulated cation current.	transcription
60422	4	335592	7	NULL	NULL	0	NULL	MeSATP	Chemical		stimulate					cation current	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_46_29080_s_7	8910562	Although injection of oocytes with either GDPbetaS (guanyl-5 -yl thiophosphate) or GTPgammaS (guanosine 5 -3- O-(thio)triphosphate) resulted in loss of adenine nucleotide-promoted Cl  channel activation, neither guanine nucleotide altered the 2MeSATP-stimulated cation current.	transcription
60423	5	335592	7	NULL	NULL	0	NULL	guanine nucleotide	NucleicAcid		does not alter					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_46_29080_s_7	8910562	Although injection of oocytes with either GDPbetaS (guanyl-5 -yl thiophosphate) or GTPgammaS (guanosine 5 -3- O-(thio)triphosphate) resulted in loss of adenine nucleotide-promoted Cl  channel activation, neither guanine nucleotide altered the 2MeSATP-stimulated cation current.	transcription
60424	6	335592	7	NULL	NULL	0	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_46_29080_s_7	8910562	Although injection of oocytes with either GDPbetaS (guanyl-5 -yl thiophosphate) or GTPgammaS (guanosine 5 -3- O-(thio)triphosphate) resulted in loss of adenine nucleotide-promoted Cl  channel activation, neither guanine nucleotide altered the 2MeSATP-stimulated cation current.	transcription
56502	1	335593	5	NULL	NULL	0	NULL	adenine			interacts with			methyl group at position N6		glucocorticoid receptor			Val-482		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_17_11679_s_219	10206981	This is probably related to the fact that the methyl group at position  N6 of adenine can mimic the 5''-methyl group of the thymine ( i.e. establish hydrophobic interaction with residue Val-482 of the glucocorticoid receptor) ( 47) and enables strong specific interaction of the GR with the major groove, although the positions of these methyl groups differ in the major groove ( 29).	transcription
60426	1	335593	7	NULL	NULL	0	NULL	adenine	Chemical	methyl group at position N6	interacts with		hydrophobically		 	glucocorticoid receptor	GP		residue Val-482		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_17_11679_s_219	10206981	This is probably related to the fact that the methyl group at position  N6 of adenine can mimic the 5''-methyl group of the thymine ( i.e. establish hydrophobic interaction with residue Val-482 of the glucocorticoid receptor) ( 47) and enables strong specific interaction of the GR with the major groove, although the positions of these methyl groups differ in the major groove ( 29).	transcription
60428	2	335593	7	NULL	NULL	0	NULL	thymine	Chemical	5''-methyl group of	interacts with		hydrophobically			glucocorticoid receptor	GP		residue Val-482		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_17_11679_s_219	10206981	This is probably related to the fact that the methyl group at position  N6 of adenine can mimic the 5''-methyl group of the thymine ( i.e. establish hydrophobic interaction with residue Val-482 of the glucocorticoid receptor) ( 47) and enables strong specific interaction of the GR with the major groove, although the positions of these methyl groups differ in the major groove ( 29).	transcription
60430	3	335593	7	NULL	NULL	0	NULL	adenine	Chemical	methyl group at position N6 of	mimic					thymine	Chemical	5''-methyl group of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_17_11679_s_219	10206981	This is probably related to the fact that the methyl group at position  N6 of adenine can mimic the 5''-methyl group of the thymine ( i.e. establish hydrophobic interaction with residue Val-482 of the glucocorticoid receptor) ( 47) and enables strong specific interaction of the GR with the major groove, although the positions of these methyl groups differ in the major groove ( 29).	transcription
60432	4	335593	7	NULL	NULL	0	NULL	GR	GP		interacts with		strongly;;specifically							major groove	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_17_11679_s_219	10206981	This is probably related to the fact that the methyl group at position  N6 of adenine can mimic the 5''-methyl group of the thymine ( i.e. establish hydrophobic interaction with residue Val-482 of the glucocorticoid receptor) ( 47) and enables strong specific interaction of the GR with the major groove, although the positions of these methyl groups differ in the major groove ( 29).	transcription
60433	5	335593	7	NULL	NULL	0	NULL	adenine	Chemical	methyl group at position N6 of	enables					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_17_11679_s_219	10206981	This is probably related to the fact that the methyl group at position  N6 of adenine can mimic the 5''-methyl group of the thymine ( i.e. establish hydrophobic interaction with residue Val-482 of the glucocorticoid receptor) ( 47) and enables strong specific interaction of the GR with the major groove, although the positions of these methyl groups differ in the major groove ( 29).	transcription
60434	6	335593	7	NULL	NULL	0	NULL	thymine	Chemical	5''-methyl group of	enables					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_17_11679_s_219	10206981	This is probably related to the fact that the methyl group at position  N6 of adenine can mimic the 5''-methyl group of the thymine ( i.e. establish hydrophobic interaction with residue Val-482 of the glucocorticoid receptor) ( 47) and enables strong specific interaction of the GR with the major groove, although the positions of these methyl groups differ in the major groove ( 29).	transcription
55414	1	335594	5	NULL	NULL	0	NULL	PHS			does not inhibit					uracil		transport of			NULL	nitrogen-repressing condition	0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_190	9446592	PHS did not inhibit uracil or adenine transport under nitrogen-repressing (ammonia ions in the culture medium), partially nitrogen-repressing (PYED medium), or nitrogen-derepressing (proline in the culture medium) conditions (Figs.  1 and  5), indicating that PHS does not affect these two families of major facilitator superfamily of membrane-bound transporters.	transcription
55416	2	335594	5	NULL	NULL	0	NULL	PHS			does not inhibit					adenine		transport of			NULL	nitrogen-repressing condition	0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_190	9446592	PHS did not inhibit uracil or adenine transport under nitrogen-repressing (ammonia ions in the culture medium), partially nitrogen-repressing (PYED medium), or nitrogen-derepressing (proline in the culture medium) conditions (Figs.  1 and  5), indicating that PHS does not affect these two families of major facilitator superfamily of membrane-bound transporters.	transcription
55418	3	335594	5	NULL	NULL	0	NULL	PHS			does not inhibit					uracil		transport of			NULL	partially nitrogen-repressing condition	0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_190	9446592	PHS did not inhibit uracil or adenine transport under nitrogen-repressing (ammonia ions in the culture medium), partially nitrogen-repressing (PYED medium), or nitrogen-derepressing (proline in the culture medium) conditions (Figs.  1 and  5), indicating that PHS does not affect these two families of major facilitator superfamily of membrane-bound transporters.	transcription
55419	4	335594	5	NULL	NULL	0	NULL	PHS			does not inhibit					adenine		transport of			NULL	partially nitrogen-repressing condition	0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_190	9446592	PHS did not inhibit uracil or adenine transport under nitrogen-repressing (ammonia ions in the culture medium), partially nitrogen-repressing (PYED medium), or nitrogen-derepressing (proline in the culture medium) conditions (Figs.  1 and  5), indicating that PHS does not affect these two families of major facilitator superfamily of membrane-bound transporters.	transcription
55421	5	335594	5	NULL	NULL	0	NULL	PHS			does not inhibit					uracil		transport of			NULL	nitrogen-derepressing condition	0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_190	9446592	PHS did not inhibit uracil or adenine transport under nitrogen-repressing (ammonia ions in the culture medium), partially nitrogen-repressing (PYED medium), or nitrogen-derepressing (proline in the culture medium) conditions (Figs.  1 and  5), indicating that PHS does not affect these two families of major facilitator superfamily of membrane-bound transporters.	transcription
55422	6	335594	5	NULL	NULL	0	NULL	PHS			does not inhibit					adenine		transport of			NULL	nitrogen-derepressing condition	0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_190	9446592	PHS did not inhibit uracil or adenine transport under nitrogen-repressing (ammonia ions in the culture medium), partially nitrogen-repressing (PYED medium), or nitrogen-derepressing (proline in the culture medium) conditions (Figs.  1 and  5), indicating that PHS does not affect these two families of major facilitator superfamily of membrane-bound transporters.	transcription
60435	1	335594	7	NULL	NULL	0	NULL	PHS	Chemical		does not inhibit					uracil	Chemical	transport of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_190	9446592	PHS did not inhibit uracil or adenine transport under nitrogen-repressing (ammonia ions in the culture medium), partially nitrogen-repressing (PYED medium), or nitrogen-derepressing (proline in the culture medium) conditions (Figs.  1 and  5), indicating that PHS does not affect these two families of major facilitator superfamily of membrane-bound transporters.	transcription
60436	2	335594	7	NULL	NULL	0	NULL	PHS	Chemical		does not inhibit					adenine	Chemical	transport of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_190	9446592	PHS did not inhibit uracil or adenine transport under nitrogen-repressing (ammonia ions in the culture medium), partially nitrogen-repressing (PYED medium), or nitrogen-derepressing (proline in the culture medium) conditions (Figs.  1 and  5), indicating that PHS does not affect these two families of major facilitator superfamily of membrane-bound transporters.	transcription
60437	3	335594	7	NULL	NULL	0	NULL	statement 1	Process		occur upon					nitrogen	Chemical	repressing			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_190	9446592	PHS did not inhibit uracil or adenine transport under nitrogen-repressing (ammonia ions in the culture medium), partially nitrogen-repressing (PYED medium), or nitrogen-derepressing (proline in the culture medium) conditions (Figs.  1 and  5), indicating that PHS does not affect these two families of major facilitator superfamily of membrane-bound transporters.	transcription
60438	4	335594	7	NULL	NULL	0	NULL	statement 2	Process		occur upon					nitrogen 	Chemical	repressing			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_190	9446592	PHS did not inhibit uracil or adenine transport under nitrogen-repressing (ammonia ions in the culture medium), partially nitrogen-repressing (PYED medium), or nitrogen-derepressing (proline in the culture medium) conditions (Figs.  1 and  5), indicating that PHS does not affect these two families of major facilitator superfamily of membrane-bound transporters.	transcription
60439	5	335594	7	NULL	NULL	0	NULL	statement 1	Process		occur upon					 nitrogen	Chemical	partially repressing			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_190	9446592	PHS did not inhibit uracil or adenine transport under nitrogen-repressing (ammonia ions in the culture medium), partially nitrogen-repressing (PYED medium), or nitrogen-derepressing (proline in the culture medium) conditions (Figs.  1 and  5), indicating that PHS does not affect these two families of major facilitator superfamily of membrane-bound transporters.	transcription
60440	6	335594	7	NULL	NULL	0	NULL	statement 2	Process		occur upon					nitrogen	Chemical	partially repressing			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_190	9446592	PHS did not inhibit uracil or adenine transport under nitrogen-repressing (ammonia ions in the culture medium), partially nitrogen-repressing (PYED medium), or nitrogen-derepressing (proline in the culture medium) conditions (Figs.  1 and  5), indicating that PHS does not affect these two families of major facilitator superfamily of membrane-bound transporters.	transcription
60441	7	335594	7	NULL	NULL	0	NULL	statement 1	Process		occur upon					nitrogen	Chemical	derepressing			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_190	9446592	PHS did not inhibit uracil or adenine transport under nitrogen-repressing (ammonia ions in the culture medium), partially nitrogen-repressing (PYED medium), or nitrogen-derepressing (proline in the culture medium) conditions (Figs.  1 and  5), indicating that PHS does not affect these two families of major facilitator superfamily of membrane-bound transporters.	transcription
60442	8	335594	7	NULL	NULL	0	NULL	statement 2	Process		occur upon					nitrogen	Chemical	derepressing			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2829_s_190	9446592	PHS did not inhibit uracil or adenine transport under nitrogen-repressing (ammonia ions in the culture medium), partially nitrogen-repressing (PYED medium), or nitrogen-derepressing (proline in the culture medium) conditions (Figs.  1 and  5), indicating that PHS does not affect these two families of major facilitator superfamily of membrane-bound transporters.	transcription
55423	1	335595	5	NULL	NULL	0	NULL	DnaA protein			initiates					chromosomal DNA		replication of;;Escherichia coli			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_33_20847_s_11	9694830	DnaA protein, the initiator of chromosomal DNA replication in  Escherichia coli ( 1-4), has a high affinity for adenine nucleotides; the ATP-binding form of DnaA protein is active, whereas the ADP-binding form is inactive in an  oriC DNA replication system  in vitro ( 5).	transcription
55424	2	335595	5	NULL	NULL	0	NULL	DnaA protein			has affinity for		high			adenine nucleotides					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_33_20847_s_11	9694830	DnaA protein, the initiator of chromosomal DNA replication in  Escherichia coli ( 1-4), has a high affinity for adenine nucleotides; the ATP-binding form of DnaA protein is active, whereas the ADP-binding form is inactive in an  oriC DNA replication system  in vitro ( 5).	transcription
55425	3	335595	5	NULL	NULL	0	NULL	DnaA protein			bind					ATP					NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_33_20847_s_11	9694830	DnaA protein, the initiator of chromosomal DNA replication in  Escherichia coli ( 1-4), has a high affinity for adenine nucleotides; the ATP-binding form of DnaA protein is active, whereas the ADP-binding form is inactive in an  oriC DNA replication system  in vitro ( 5).	transcription
55426	4	335595	5	NULL	NULL	0	NULL	statement 3			is active in					oriC DNA replication system					NULL	in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_273_33_20847_s_11	9694830	DnaA protein, the initiator of chromosomal DNA replication in  Escherichia coli ( 1-4), has a high affinity for adenine nucleotides; the ATP-binding form of DnaA protein is active, whereas the ADP-binding form is inactive in an  oriC DNA replication system  in vitro ( 5).	transcription
55427	5	335595	5	NULL	NULL	0	NULL	DnaA protein			bind					ADP					NULL	in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_33_20847_s_11	9694830	DnaA protein, the initiator of chromosomal DNA replication in  Escherichia coli ( 1-4), has a high affinity for adenine nucleotides; the ATP-binding form of DnaA protein is active, whereas the ADP-binding form is inactive in an  oriC DNA replication system  in vitro ( 5).	transcription
55428	6	335595	5	NULL	NULL	0	NULL	statement 5			is inactivate in					oriC DNA replication system					NULL	in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_273_33_20847_s_11	9694830	DnaA protein, the initiator of chromosomal DNA replication in  Escherichia coli ( 1-4), has a high affinity for adenine nucleotides; the ATP-binding form of DnaA protein is active, whereas the ADP-binding form is inactive in an  oriC DNA replication system  in vitro ( 5).	transcription
60443	1	335595	7	NULL	NULL	0	NULL	DnaA protein	GP		is the initiator of					chromosomal DNA	NucleicAcid	replication of			NULL	Escherichia coli 	0	NULL	NULL	NULL	gw60_jbiolchem_273_33_20847_s_11	9694830	DnaA protein, the initiator of chromosomal DNA replication in  Escherichia coli ( 1-4), has a high affinity for adenine nucleotides; the ATP-binding form of DnaA protein is active, whereas the ADP-binding form is inactive in an  oriC DNA replication system  in vitro ( 5).	transcription
60444	2	335595	7	NULL	NULL	0	NULL	DnaA protein	GP		high affinity for					adenine nucleotides	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_33_20847_s_11	9694830	DnaA protein, the initiator of chromosomal DNA replication in  Escherichia coli ( 1-4), has a high affinity for adenine nucleotides; the ATP-binding form of DnaA protein is active, whereas the ADP-binding form is inactive in an  oriC DNA replication system  in vitro ( 5).	transcription
60445	3	335595	7	NULL	NULL	0	NULL	DnaA protein	GP		bind					ATP	Chemical				NULL	oriC DNA replication system in vitro	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_33_20847_s_11	9694830	DnaA protein, the initiator of chromosomal DNA replication in  Escherichia coli ( 1-4), has a high affinity for adenine nucleotides; the ATP-binding form of DnaA protein is active, whereas the ADP-binding form is inactive in an  oriC DNA replication system  in vitro ( 5).	transcription
60446	4	335595	7	NULL	NULL	0	NULL	DnaA protein	GP		bind					ADP	Chemical				NULL	oriC DNA replication system in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_273_33_20847_s_11	9694830	DnaA protein, the initiator of chromosomal DNA replication in  Escherichia coli ( 1-4), has a high affinity for adenine nucleotides; the ATP-binding form of DnaA protein is active, whereas the ADP-binding form is inactive in an  oriC DNA replication system  in vitro ( 5).	transcription
60447	5	335595	7	NULL	NULL	0	NULL	statement 3	Process		is					active	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_33_20847_s_11	9694830	DnaA protein, the initiator of chromosomal DNA replication in  Escherichia coli ( 1-4), has a high affinity for adenine nucleotides; the ATP-binding form of DnaA protein is active, whereas the ADP-binding form is inactive in an  oriC DNA replication system  in vitro ( 5).	transcription
60448	6	335595	7	NULL	NULL	0	NULL	statement 4	Process		is					inactive	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_33_20847_s_11	9694830	DnaA protein, the initiator of chromosomal DNA replication in  Escherichia coli ( 1-4), has a high affinity for adenine nucleotides; the ATP-binding form of DnaA protein is active, whereas the ADP-binding form is inactive in an  oriC DNA replication system  in vitro ( 5).	transcription
55429	1	335596	5	NULL	NULL	0	NULL	iodotubercidine			is an inhibitor of					adenosine kinase					NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_988_s_39	10565815	The probes were connected to a CMA/100 microinfusion pump (Carnergie Medicine, Stockholm, Sweden) and were perfused with isotonic saline solution with heparin (30 U/ml) containing iodotubercidine (10 muM), an inhibitor of adenosine kinase, and  erythro-9-(2-hydroxy-3-nonyl)adenine (EHNA) (100 muM), an inhibitor of adenosine deaminase, at a rate of 5 mul/min.	transcription
55430	2	335596	5	NULL	NULL	0	NULL	EHNA			is					erythro-9-(2-hydroxy-3-nonyl)adenine					NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_988_s_39	10565815	The probes were connected to a CMA/100 microinfusion pump (Carnergie Medicine, Stockholm, Sweden) and were perfused with isotonic saline solution with heparin (30 U/ml) containing iodotubercidine (10 muM), an inhibitor of adenosine kinase, and  erythro-9-(2-hydroxy-3-nonyl)adenine (EHNA) (100 muM), an inhibitor of adenosine deaminase, at a rate of 5 mul/min.	transcription
55431	3	335596	5	NULL	NULL	0	NULL	EHNA			inhibit					adenosine deaminase					NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_988_s_39	10565815	The probes were connected to a CMA/100 microinfusion pump (Carnergie Medicine, Stockholm, Sweden) and were perfused with isotonic saline solution with heparin (30 U/ml) containing iodotubercidine (10 muM), an inhibitor of adenosine kinase, and  erythro-9-(2-hydroxy-3-nonyl)adenine (EHNA) (100 muM), an inhibitor of adenosine deaminase, at a rate of 5 mul/min.	transcription
60449	1	335596	7	NULL	NULL	0	NULL	iodotubercidine	Chemical		is an inhibitor of					adenosine kinase	GP				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_988_s_39	10565815	The probes were connected to a CMA/100 microinfusion pump (Carnergie Medicine, Stockholm, Sweden) and were perfused with isotonic saline solution with heparin (30 U/ml) containing iodotubercidine (10 muM), an inhibitor of adenosine kinase, and  erythro-9-(2-hydroxy-3-nonyl)adenine (EHNA) (100 muM), an inhibitor of adenosine deaminase, at a rate of 5 mul/min.	transcription
60450	2	335596	7	NULL	NULL	0	NULL	EHNA	Chemical		is an inhibitor of					adenosine kinase	GP				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_988_s_39	10565815	The probes were connected to a CMA/100 microinfusion pump (Carnergie Medicine, Stockholm, Sweden) and were perfused with isotonic saline solution with heparin (30 U/ml) containing iodotubercidine (10 muM), an inhibitor of adenosine kinase, and  erythro-9-(2-hydroxy-3-nonyl)adenine (EHNA) (100 muM), an inhibitor of adenosine deaminase, at a rate of 5 mul/min.	transcription
60451	3	335596	7	NULL	NULL	0	NULL	EHNA	Chemical		is					erythro-9-(2-hydroxy-3-nonyl)adenine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_291_3_988_s_39	10565815	The probes were connected to a CMA/100 microinfusion pump (Carnergie Medicine, Stockholm, Sweden) and were perfused with isotonic saline solution with heparin (30 U/ml) containing iodotubercidine (10 muM), an inhibitor of adenosine kinase, and  erythro-9-(2-hydroxy-3-nonyl)adenine (EHNA) (100 muM), an inhibitor of adenosine deaminase, at a rate of 5 mul/min.	transcription
55432	1	335597	5	NULL	NULL	0	NULL	Escherichia coli			is a type of					enteric bacterium					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_16_4116_s_17	9696758	In the enteric bacterium  Escherichia coli, three methyltransferases are present: (i) Dam (DNA adenine methyltransferase), creating N6-methyladenosine in the specific target sequence 5''-GmATC-3''; (ii) Dcm (DNA cytosine methyltransferase), leading to an internal C5-methylcytosine in the specific target sequence 5''-CmC(A/T)GG-3''; and (iii) methyltransferase M.   EcoK, modifying the second adenine in the sequence AmAC(N6)GTCG, which is specifically recognized as an unmethylated sequence by restriction endonuclease  EcoK, which is part of the host-specific restriction-modification (R-M) system (for a review, see reference  22).	transcription
55433	2	335597	5	NULL	NULL	0	NULL	Dam			is present in					Escherichia coli					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_16_4116_s_17	9696758	In the enteric bacterium  Escherichia coli, three methyltransferases are present: (i) Dam (DNA adenine methyltransferase), creating N6-methyladenosine in the specific target sequence 5''-GmATC-3''; (ii) Dcm (DNA cytosine methyltransferase), leading to an internal C5-methylcytosine in the specific target sequence 5''-CmC(A/T)GG-3''; and (iii) methyltransferase M.   EcoK, modifying the second adenine in the sequence AmAC(N6)GTCG, which is specifically recognized as an unmethylated sequence by restriction endonuclease  EcoK, which is part of the host-specific restriction-modification (R-M) system (for a review, see reference  22).	transcription
55434	3	335597	5	NULL	NULL	0	NULL	Dcm			is present in					Escherichia coli					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_16_4116_s_17	9696758	In the enteric bacterium  Escherichia coli, three methyltransferases are present: (i) Dam (DNA adenine methyltransferase), creating N6-methyladenosine in the specific target sequence 5''-GmATC-3''; (ii) Dcm (DNA cytosine methyltransferase), leading to an internal C5-methylcytosine in the specific target sequence 5''-CmC(A/T)GG-3''; and (iii) methyltransferase M.   EcoK, modifying the second adenine in the sequence AmAC(N6)GTCG, which is specifically recognized as an unmethylated sequence by restriction endonuclease  EcoK, which is part of the host-specific restriction-modification (R-M) system (for a review, see reference  22).	transcription
55435	4	335597	5	NULL	NULL	0	NULL	M. EcoK			is present in					Escherichia coli					NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_16_4116_s_17	9696758	In the enteric bacterium  Escherichia coli, three methyltransferases are present: (i) Dam (DNA adenine methyltransferase), creating N6-methyladenosine in the specific target sequence 5''-GmATC-3''; (ii) Dcm (DNA cytosine methyltransferase), leading to an internal C5-methylcytosine in the specific target sequence 5''-CmC(A/T)GG-3''; and (iii) methyltransferase M.   EcoK, modifying the second adenine in the sequence AmAC(N6)GTCG, which is specifically recognized as an unmethylated sequence by restriction endonuclease  EcoK, which is part of the host-specific restriction-modification (R-M) system (for a review, see reference  22).	transcription
55436	5	335597	5	NULL	NULL	0	NULL	Dam			is					DNA adenine methyltransferase					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_16_4116_s_17	9696758	In the enteric bacterium  Escherichia coli, three methyltransferases are present: (i) Dam (DNA adenine methyltransferase), creating N6-methyladenosine in the specific target sequence 5''-GmATC-3''; (ii) Dcm (DNA cytosine methyltransferase), leading to an internal C5-methylcytosine in the specific target sequence 5''-CmC(A/T)GG-3''; and (iii) methyltransferase M.   EcoK, modifying the second adenine in the sequence AmAC(N6)GTCG, which is specifically recognized as an unmethylated sequence by restriction endonuclease  EcoK, which is part of the host-specific restriction-modification (R-M) system (for a review, see reference  22).	transcription
55437	6	335597	5	NULL	NULL	0	NULL	Dcm			is					DNA cytosine methyltransferase					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_16_4116_s_17	9696758	In the enteric bacterium  Escherichia coli, three methyltransferases are present: (i) Dam (DNA adenine methyltransferase), creating N6-methyladenosine in the specific target sequence 5''-GmATC-3''; (ii) Dcm (DNA cytosine methyltransferase), leading to an internal C5-methylcytosine in the specific target sequence 5''-CmC(A/T)GG-3''; and (iii) methyltransferase M.   EcoK, modifying the second adenine in the sequence AmAC(N6)GTCG, which is specifically recognized as an unmethylated sequence by restriction endonuclease  EcoK, which is part of the host-specific restriction-modification (R-M) system (for a review, see reference  22).	transcription
55438	7	335597	5	NULL	NULL	0	NULL	N6-methyladenosine			is created in							specific;;target sequence		5''-GmATC-3''	NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_16_4116_s_17	9696758	In the enteric bacterium  Escherichia coli, three methyltransferases are present: (i) Dam (DNA adenine methyltransferase), creating N6-methyladenosine in the specific target sequence 5''-GmATC-3''; (ii) Dcm (DNA cytosine methyltransferase), leading to an internal C5-methylcytosine in the specific target sequence 5''-CmC(A/T)GG-3''; and (iii) methyltransferase M.   EcoK, modifying the second adenine in the sequence AmAC(N6)GTCG, which is specifically recognized as an unmethylated sequence by restriction endonuclease  EcoK, which is part of the host-specific restriction-modification (R-M) system (for a review, see reference  22).	transcription
55439	8	335597	5	NULL	NULL	0	NULL	Dam			is required for					statement 7					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_16_4116_s_17	9696758	In the enteric bacterium  Escherichia coli, three methyltransferases are present: (i) Dam (DNA adenine methyltransferase), creating N6-methyladenosine in the specific target sequence 5''-GmATC-3''; (ii) Dcm (DNA cytosine methyltransferase), leading to an internal C5-methylcytosine in the specific target sequence 5''-CmC(A/T)GG-3''; and (iii) methyltransferase M.   EcoK, modifying the second adenine in the sequence AmAC(N6)GTCG, which is specifically recognized as an unmethylated sequence by restriction endonuclease  EcoK, which is part of the host-specific restriction-modification (R-M) system (for a review, see reference  22).	transcription
55440	9	335597	5	NULL	NULL	0	NULL	C5-methylcytosine		internal	is created in							specific;;target sequence		5''-CmC(A/T)GG-3''	NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_16_4116_s_17	9696758	In the enteric bacterium  Escherichia coli, three methyltransferases are present: (i) Dam (DNA adenine methyltransferase), creating N6-methyladenosine in the specific target sequence 5''-GmATC-3''; (ii) Dcm (DNA cytosine methyltransferase), leading to an internal C5-methylcytosine in the specific target sequence 5''-CmC(A/T)GG-3''; and (iii) methyltransferase M.   EcoK, modifying the second adenine in the sequence AmAC(N6)GTCG, which is specifically recognized as an unmethylated sequence by restriction endonuclease  EcoK, which is part of the host-specific restriction-modification (R-M) system (for a review, see reference  22).	transcription
55441	10	335597	5	NULL	NULL	0	NULL	Dcm			is required for					statement 9					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_16_4116_s_17	9696758	In the enteric bacterium  Escherichia coli, three methyltransferases are present: (i) Dam (DNA adenine methyltransferase), creating N6-methyladenosine in the specific target sequence 5''-GmATC-3''; (ii) Dcm (DNA cytosine methyltransferase), leading to an internal C5-methylcytosine in the specific target sequence 5''-CmC(A/T)GG-3''; and (iii) methyltransferase M.   EcoK, modifying the second adenine in the sequence AmAC(N6)GTCG, which is specifically recognized as an unmethylated sequence by restriction endonuclease  EcoK, which is part of the host-specific restriction-modification (R-M) system (for a review, see reference  22).	transcription
55442	11	335597	5	NULL	NULL	0	NULL	adenine			is modified in									AmAC(N6)GTCG	NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_16_4116_s_17	9696758	In the enteric bacterium  Escherichia coli, three methyltransferases are present: (i) Dam (DNA adenine methyltransferase), creating N6-methyladenosine in the specific target sequence 5''-GmATC-3''; (ii) Dcm (DNA cytosine methyltransferase), leading to an internal C5-methylcytosine in the specific target sequence 5''-CmC(A/T)GG-3''; and (iii) methyltransferase M.   EcoK, modifying the second adenine in the sequence AmAC(N6)GTCG, which is specifically recognized as an unmethylated sequence by restriction endonuclease  EcoK, which is part of the host-specific restriction-modification (R-M) system (for a review, see reference  22).	transcription
55443	12	335597	5	NULL	NULL	0	NULL	M. EcoK			is required for					statement 11					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_16_4116_s_17	9696758	In the enteric bacterium  Escherichia coli, three methyltransferases are present: (i) Dam (DNA adenine methyltransferase), creating N6-methyladenosine in the specific target sequence 5''-GmATC-3''; (ii) Dcm (DNA cytosine methyltransferase), leading to an internal C5-methylcytosine in the specific target sequence 5''-CmC(A/T)GG-3''; and (iii) methyltransferase M.   EcoK, modifying the second adenine in the sequence AmAC(N6)GTCG, which is specifically recognized as an unmethylated sequence by restriction endonuclease  EcoK, which is part of the host-specific restriction-modification (R-M) system (for a review, see reference  22).	transcription
55444	13	335597	5	NULL	NULL	0	NULL				is recognized as		specifically		AmAC(N6)GTCG	unmethylated sequence					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_16_4116_s_17	9696758	In the enteric bacterium  Escherichia coli, three methyltransferases are present: (i) Dam (DNA adenine methyltransferase), creating N6-methyladenosine in the specific target sequence 5''-GmATC-3''; (ii) Dcm (DNA cytosine methyltransferase), leading to an internal C5-methylcytosine in the specific target sequence 5''-CmC(A/T)GG-3''; and (iii) methyltransferase M.   EcoK, modifying the second adenine in the sequence AmAC(N6)GTCG, which is specifically recognized as an unmethylated sequence by restriction endonuclease  EcoK, which is part of the host-specific restriction-modification (R-M) system (for a review, see reference  22).	transcription
55445	14	335597	5	NULL	NULL	0	NULL	EcoK			is a type of					endonuclease					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_16_4116_s_17	9696758	In the enteric bacterium  Escherichia coli, three methyltransferases are present: (i) Dam (DNA adenine methyltransferase), creating N6-methyladenosine in the specific target sequence 5''-GmATC-3''; (ii) Dcm (DNA cytosine methyltransferase), leading to an internal C5-methylcytosine in the specific target sequence 5''-CmC(A/T)GG-3''; and (iii) methyltransferase M.   EcoK, modifying the second adenine in the sequence AmAC(N6)GTCG, which is specifically recognized as an unmethylated sequence by restriction endonuclease  EcoK, which is part of the host-specific restriction-modification (R-M) system (for a review, see reference  22).	transcription
55446	15	335597	5	NULL	NULL	0	NULL	EcoK			is required for					statement 13					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_16_4116_s_17	9696758	In the enteric bacterium  Escherichia coli, three methyltransferases are present: (i) Dam (DNA adenine methyltransferase), creating N6-methyladenosine in the specific target sequence 5''-GmATC-3''; (ii) Dcm (DNA cytosine methyltransferase), leading to an internal C5-methylcytosine in the specific target sequence 5''-CmC(A/T)GG-3''; and (iii) methyltransferase M.   EcoK, modifying the second adenine in the sequence AmAC(N6)GTCG, which is specifically recognized as an unmethylated sequence by restriction endonuclease  EcoK, which is part of the host-specific restriction-modification (R-M) system (for a review, see reference  22).	transcription
55447	16	335597	5	NULL	NULL	0	NULL	R-M system			is					restriction-modification system					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_16_4116_s_17	9696758	In the enteric bacterium  Escherichia coli, three methyltransferases are present: (i) Dam (DNA adenine methyltransferase), creating N6-methyladenosine in the specific target sequence 5''-GmATC-3''; (ii) Dcm (DNA cytosine methyltransferase), leading to an internal C5-methylcytosine in the specific target sequence 5''-CmC(A/T)GG-3''; and (iii) methyltransferase M.   EcoK, modifying the second adenine in the sequence AmAC(N6)GTCG, which is specifically recognized as an unmethylated sequence by restriction endonuclease  EcoK, which is part of the host-specific restriction-modification (R-M) system (for a review, see reference  22).	transcription
55448	17	335597	5	NULL	NULL	0	NULL	R-M system			is specific to					host					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_16_4116_s_17	9696758	In the enteric bacterium  Escherichia coli, three methyltransferases are present: (i) Dam (DNA adenine methyltransferase), creating N6-methyladenosine in the specific target sequence 5''-GmATC-3''; (ii) Dcm (DNA cytosine methyltransferase), leading to an internal C5-methylcytosine in the specific target sequence 5''-CmC(A/T)GG-3''; and (iii) methyltransferase M.   EcoK, modifying the second adenine in the sequence AmAC(N6)GTCG, which is specifically recognized as an unmethylated sequence by restriction endonuclease  EcoK, which is part of the host-specific restriction-modification (R-M) system (for a review, see reference  22).	transcription
55449	18	335597	5	NULL	NULL	0	NULL	statement 13			is a part of					R-M system					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_16_4116_s_17	9696758	In the enteric bacterium  Escherichia coli, three methyltransferases are present: (i) Dam (DNA adenine methyltransferase), creating N6-methyladenosine in the specific target sequence 5''-GmATC-3''; (ii) Dcm (DNA cytosine methyltransferase), leading to an internal C5-methylcytosine in the specific target sequence 5''-CmC(A/T)GG-3''; and (iii) methyltransferase M.   EcoK, modifying the second adenine in the sequence AmAC(N6)GTCG, which is specifically recognized as an unmethylated sequence by restriction endonuclease  EcoK, which is part of the host-specific restriction-modification (R-M) system (for a review, see reference  22).	transcription
60452	1	335597	7	NULL	NULL	0	NULL	Dam	GP		creates					N6-methyladenosine 	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_16_4116_s_17	9696758	In the enteric bacterium  Escherichia coli, three methyltransferases are present: (i) Dam (DNA adenine methyltransferase), creating N6-methyladenosine in the specific target sequence 5''-GmATC-3''; (ii) Dcm (DNA cytosine methyltransferase), leading to an internal C5-methylcytosine in the specific target sequence 5''-CmC(A/T)GG-3''; and (iii) methyltransferase M.   EcoK, modifying the second adenine in the sequence AmAC(N6)GTCG, which is specifically recognized as an unmethylated sequence by restriction endonuclease  EcoK, which is part of the host-specific restriction-modification (R-M) system (for a review, see reference  22).	transcription
60453	2	335597	7	NULL	NULL	0	NULL	statement 1	Process		occur in							target sequence		5''-GmATC-3''	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_16_4116_s_17	9696758	In the enteric bacterium  Escherichia coli, three methyltransferases are present: (i) Dam (DNA adenine methyltransferase), creating N6-methyladenosine in the specific target sequence 5''-GmATC-3''; (ii) Dcm (DNA cytosine methyltransferase), leading to an internal C5-methylcytosine in the specific target sequence 5''-CmC(A/T)GG-3''; and (iii) methyltransferase M.   EcoK, modifying the second adenine in the sequence AmAC(N6)GTCG, which is specifically recognized as an unmethylated sequence by restriction endonuclease  EcoK, which is part of the host-specific restriction-modification (R-M) system (for a review, see reference  22).	transcription
60454	3	335597	7	NULL	NULL	0	NULL	Dcm	GP		leads to					C5-methylcytosine	Chemical	internal			NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_16_4116_s_17	9696758	In the enteric bacterium  Escherichia coli, three methyltransferases are present: (i) Dam (DNA adenine methyltransferase), creating N6-methyladenosine in the specific target sequence 5''-GmATC-3''; (ii) Dcm (DNA cytosine methyltransferase), leading to an internal C5-methylcytosine in the specific target sequence 5''-CmC(A/T)GG-3''; and (iii) methyltransferase M.   EcoK, modifying the second adenine in the sequence AmAC(N6)GTCG, which is specifically recognized as an unmethylated sequence by restriction endonuclease  EcoK, which is part of the host-specific restriction-modification (R-M) system (for a review, see reference  22).	transcription
60455	4	335597	7	NULL	NULL	0	NULL	statement 3	Process		occur in							target sequence		5''-CmC(A/T)GG-3''	NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_16_4116_s_17	9696758	In the enteric bacterium  Escherichia coli, three methyltransferases are present: (i) Dam (DNA adenine methyltransferase), creating N6-methyladenosine in the specific target sequence 5''-GmATC-3''; (ii) Dcm (DNA cytosine methyltransferase), leading to an internal C5-methylcytosine in the specific target sequence 5''-CmC(A/T)GG-3''; and (iii) methyltransferase M.   EcoK, modifying the second adenine in the sequence AmAC(N6)GTCG, which is specifically recognized as an unmethylated sequence by restriction endonuclease  EcoK, which is part of the host-specific restriction-modification (R-M) system (for a review, see reference  22).	transcription
60456	5	335597	7	NULL	NULL	0	NULL	M. EcoK	GP		modifies							second adenine in		AmAC(N6)GTCG	NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_180_16_4116_s_17	9696758	In the enteric bacterium  Escherichia coli, three methyltransferases are present: (i) Dam (DNA adenine methyltransferase), creating N6-methyladenosine in the specific target sequence 5''-GmATC-3''; (ii) Dcm (DNA cytosine methyltransferase), leading to an internal C5-methylcytosine in the specific target sequence 5''-CmC(A/T)GG-3''; and (iii) methyltransferase M.   EcoK, modifying the second adenine in the sequence AmAC(N6)GTCG, which is specifically recognized as an unmethylated sequence by restriction endonuclease  EcoK, which is part of the host-specific restriction-modification (R-M) system (for a review, see reference  22).	transcription
60457	6	335597	7	NULL	NULL	0	NULL				recognized as		specifically		AmAC(N6)GTCG	unmethylated sequence					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_16_4116_s_17	9696758	In the enteric bacterium  Escherichia coli, three methyltransferases are present: (i) Dam (DNA adenine methyltransferase), creating N6-methyladenosine in the specific target sequence 5''-GmATC-3''; (ii) Dcm (DNA cytosine methyltransferase), leading to an internal C5-methylcytosine in the specific target sequence 5''-CmC(A/T)GG-3''; and (iii) methyltransferase M.   EcoK, modifying the second adenine in the sequence AmAC(N6)GTCG, which is specifically recognized as an unmethylated sequence by restriction endonuclease  EcoK, which is part of the host-specific restriction-modification (R-M) system (for a review, see reference  22).	transcription
60458	7	335597	7	NULL	NULL	0	NULL	statement 6	Process		recognized by					EcoK	GP				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_16_4116_s_17	9696758	In the enteric bacterium  Escherichia coli, three methyltransferases are present: (i) Dam (DNA adenine methyltransferase), creating N6-methyladenosine in the specific target sequence 5''-GmATC-3''; (ii) Dcm (DNA cytosine methyltransferase), leading to an internal C5-methylcytosine in the specific target sequence 5''-CmC(A/T)GG-3''; and (iii) methyltransferase M.   EcoK, modifying the second adenine in the sequence AmAC(N6)GTCG, which is specifically recognized as an unmethylated sequence by restriction endonuclease  EcoK, which is part of the host-specific restriction-modification (R-M) system (for a review, see reference  22).	transcription
60459	8	335597	7	NULL	NULL	0	NULL	EcoK	GP		is part of					host-specific restriction-modification system	Process				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_16_4116_s_17	9696758	In the enteric bacterium  Escherichia coli, three methyltransferases are present: (i) Dam (DNA adenine methyltransferase), creating N6-methyladenosine in the specific target sequence 5''-GmATC-3''; (ii) Dcm (DNA cytosine methyltransferase), leading to an internal C5-methylcytosine in the specific target sequence 5''-CmC(A/T)GG-3''; and (iii) methyltransferase M.   EcoK, modifying the second adenine in the sequence AmAC(N6)GTCG, which is specifically recognized as an unmethylated sequence by restriction endonuclease  EcoK, which is part of the host-specific restriction-modification (R-M) system (for a review, see reference  22).	transcription
60460	9	335597	7	NULL	NULL	0	NULL	EcoK	GP		is a type of					restriction endonuclease	GP				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_16_4116_s_17	9696758	In the enteric bacterium  Escherichia coli, three methyltransferases are present: (i) Dam (DNA adenine methyltransferase), creating N6-methyladenosine in the specific target sequence 5''-GmATC-3''; (ii) Dcm (DNA cytosine methyltransferase), leading to an internal C5-methylcytosine in the specific target sequence 5''-CmC(A/T)GG-3''; and (iii) methyltransferase M.   EcoK, modifying the second adenine in the sequence AmAC(N6)GTCG, which is specifically recognized as an unmethylated sequence by restriction endonuclease  EcoK, which is part of the host-specific restriction-modification (R-M) system (for a review, see reference  22).	transcription
60461	10	335597	7	NULL	NULL	0	NULL	Dam	GP		is					DNA adenine methyltransferase	GP				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_16_4116_s_17	9696758	In the enteric bacterium  Escherichia coli, three methyltransferases are present: (i) Dam (DNA adenine methyltransferase), creating N6-methyladenosine in the specific target sequence 5''-GmATC-3''; (ii) Dcm (DNA cytosine methyltransferase), leading to an internal C5-methylcytosine in the specific target sequence 5''-CmC(A/T)GG-3''; and (iii) methyltransferase M.   EcoK, modifying the second adenine in the sequence AmAC(N6)GTCG, which is specifically recognized as an unmethylated sequence by restriction endonuclease  EcoK, which is part of the host-specific restriction-modification (R-M) system (for a review, see reference  22).	transcription
60462	11	335597	7	NULL	NULL	0	NULL	Dcm	GP		is					DNA cytosine methyltransferase	GP				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_16_4116_s_17	9696758	In the enteric bacterium  Escherichia coli, three methyltransferases are present: (i) Dam (DNA adenine methyltransferase), creating N6-methyladenosine in the specific target sequence 5''-GmATC-3''; (ii) Dcm (DNA cytosine methyltransferase), leading to an internal C5-methylcytosine in the specific target sequence 5''-CmC(A/T)GG-3''; and (iii) methyltransferase M.   EcoK, modifying the second adenine in the sequence AmAC(N6)GTCG, which is specifically recognized as an unmethylated sequence by restriction endonuclease  EcoK, which is part of the host-specific restriction-modification (R-M) system (for a review, see reference  22).	transcription
60463	12	335597	7	NULL	NULL	0	NULL	M. EcoK	GP		is a type of					methyltransferase	GP				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_180_16_4116_s_17	9696758	In the enteric bacterium  Escherichia coli, three methyltransferases are present: (i) Dam (DNA adenine methyltransferase), creating N6-methyladenosine in the specific target sequence 5''-GmATC-3''; (ii) Dcm (DNA cytosine methyltransferase), leading to an internal C5-methylcytosine in the specific target sequence 5''-CmC(A/T)GG-3''; and (iii) methyltransferase M.   EcoK, modifying the second adenine in the sequence AmAC(N6)GTCG, which is specifically recognized as an unmethylated sequence by restriction endonuclease  EcoK, which is part of the host-specific restriction-modification (R-M) system (for a review, see reference  22).	transcription
55450	1	335598	5	NULL	NULL	0	NULL	GMP			is converted to					adenine nucleotides					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
55451	2	335598	5	NULL	NULL	0	NULL	statement 1			via					GMP reductase					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
55452	3	335598	5	NULL	NULL	0	NULL	GMP reductase			is encoded by					guaC gene					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
55453	4	335598	5	NULL	NULL	0	NULL	phosphoribosylpyrophosphate synthetase			is inhibited by		presumably 			ADP					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
55454	5	335598	5	NULL	NULL	0	NULL	ADP			is a type of					adenine nucleotide					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
55455	6	335598	5	NULL	NULL	0	NULL	statement 4			causes					histidine		starvation for			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
55456	7	335598	5	NULL	NULL	0	NULL	statement 4			causes					tryptophan		starvation for			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
55457	8	335598	5	NULL	NULL	0	NULL	statement 4			causes					pyrimidines		starvation for			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
55458	9	335598	5	NULL	NULL	0	NULL	PRPP			is required for					histidine		synthesis of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
55459	10	335598	5	NULL	NULL	0	NULL	PRPP			is required for					tryptophan		synthesis of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
55460	11	335598	5	NULL	NULL	0	NULL	PRPP			is required for					pyrimidines		synthesis of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
55461	12	335598	5	NULL	NULL	0	NULL	ppGpp			is					guanosine 5'',3''-bispyrophosphate					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
55462	13	335598	5	NULL	NULL	0	NULL	ppGpp			is a type of					nucleotide					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
55463	14	335598	5	NULL	NULL	0	NULL	ppGpp			is a type of					transcriptional inhibitor					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
55464	15	335598	5	NULL	NULL	0	NULL	ppGpp			is synthesized by					relA gene product					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
55465	16	335598	5	NULL	NULL	0	NULL	statement 15			in response to					amino acid		starvation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
60473	1	335598	7	NULL	NULL	0	NULL	GMP	Chemical		converted to					adenine nucleotides 	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
60474	2	335598	7	NULL	NULL	0	NULL	statement 1	Process		via					GMP reductase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
60475	3	335598	7	NULL	NULL	0	NULL	GMP reductase	GP		encoded by					guaC gene	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
60476	4	335598	7	NULL	NULL	0	NULL	ADP	Chemical		inhibit					 phosphoribosylpyrophosphate synthetase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
60477	5	335598	7	NULL	NULL	0	NULL	statement 4	Process		cause					histidine	AminoAcid	starvation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
60478	6	335598	7	NULL	NULL	0	NULL	statement 4	Process		cause					tryptophan	AminoAcid	starvation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
60479	7	335598	7	NULL	NULL	0	NULL	statement 4	Process		cause					pyrimidines	Chemical	starvation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
60482	8	335598	7	NULL	NULL	0	NULL	histidine	AminoAcid	synthesis of	require					PRPP	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
60486	9	335598	7	NULL	NULL	0	NULL	tryptophan	AminoAcid	synthesis of	require					PRPP	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
60490	10	335598	7	NULL	NULL	0	NULL	pyrimidines	Chemical	synthesis of	require					PRPP	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
60496	11	335598	7	NULL	NULL	0	NULL	ppGpp	Chemical		is a type of					transcriptional inhibitor	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
60500	12	335598	7	NULL	NULL	0	NULL	relA gene product	GP		synthesize					ppGpp	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
60501	13	335598	7	NULL	NULL	0	NULL	statement 12	Process		in response to					amino acid	AminoAcid	starvation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
60502	14	335598	7	NULL	NULL	0	NULL	ppGpp	NucleicAcid		is a type of					regulatory nucleotide	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
60503	15	335598	7	NULL	NULL	0	NULL	ppGPpp	NucleicAcid		is					guanosine 5'',3''-bispyrophosphate	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_9_5348_s_7	10026143	By isolation and characterization of guanosine-resistant derivatives of the  gsk-3 mutant, some of the crucial steps in this deleterious cascade of events were found to include the following: first, conversion of GMP to adenine nucleotides via GMP reductase, encoded by the  guaC gene; second, inhibition of phosphoribosylpyrophosphate synthetase by an adenine nucleotide, presumably ADP, causing starvation for histidine, tryptophan, and pyrimidines, all of which require PRPP for their synthesis; third, accumulation of the regulatory nucleotide guanosine 5'',3''-bispyrophosphate (ppGpp), a general transcriptional inhibitor synthesized by the  relA gene product in response to amino acid starvation.	transcription
55466	1	335603	5	NULL	NULL	0	NULL				bind			modular zinc finger domains						subsites containing a 5''-adenine	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_31_29466_s_288	11340073	Phage display selection of modular zinc finger domains that bind to subsites containing a 5''-adenine or -cytosine from our previously described finger-2 library based on the 3-finger protein C7 ( 7) failed due to the limitations imposed by Asp2 of finger 3 of this protein which makes a cross-subsite contact to the nucleotide complementary to the 5''-position of the finger-2 subsite (Fig.  1 A).	transcription
55467	2	335603	5	NULL	NULL	0	NULL				bind			modular zinc finger domains					subsites containing a 5''-cytosine		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_31_29466_s_288	11340073	Phage display selection of modular zinc finger domains that bind to subsites containing a 5''-adenine or -cytosine from our previously described finger-2 library based on the 3-finger protein C7 ( 7) failed due to the limitations imposed by Asp2 of finger 3 of this protein which makes a cross-subsite contact to the nucleotide complementary to the 5''-position of the finger-2 subsite (Fig.  1 A).	transcription
60505	1	335603	7	NULL	NULL	0	NULL			Phage	bind			modular zinc finger domain						subsites containing a 5''-adenine	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_31_29466_s_288	11340073	Phage display selection of modular zinc finger domains that bind to subsites containing a 5''-adenine or -cytosine from our previously described finger-2 library based on the 3-finger protein C7 ( 7) failed due to the limitations imposed by Asp2 of finger 3 of this protein which makes a cross-subsite contact to the nucleotide complementary to the 5''-position of the finger-2 subsite (Fig.  1 A).	transcription
60506	2	335603	7	NULL	NULL	0	NULL			Phage	bind			modular zinc finger domain						subsites containing a 5''-cytosine	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_31_29466_s_288	11340073	Phage display selection of modular zinc finger domains that bind to subsites containing a 5''-adenine or -cytosine from our previously described finger-2 library based on the 3-finger protein C7 ( 7) failed due to the limitations imposed by Asp2 of finger 3 of this protein which makes a cross-subsite contact to the nucleotide complementary to the 5''-position of the finger-2 subsite (Fig.  1 A).	transcription
55468	1	335607	5	NULL	NULL	0	NULL	complex III			is present in					electron transport chain					NULL		0	NULL	NULL	NULL	gw70_molpharmacol_70_4_1424_s_269	16849592	1) Ec targets  complex III in the electron transport chain resulting in hyperpolarization of the  mitochondrial membrane; 2) decoupling of electron transport from adenine nucleotide  transport and ATP production; 3) inhibition of ANT and ROS generation; 4) ROS stimulates  ER Ca2+ release; and 5) Ec also blocks Ca2+ influx, resulting in an ER stress response.	transcription
55469	2	335607	5	NULL	NULL	0	NULL	Ec			targets					statement 1					NULL		0	NULL	NULL	NULL	gw70_molpharmacol_70_4_1424_s_269	16849592	1) Ec targets  complex III in the electron transport chain resulting in hyperpolarization of the  mitochondrial membrane; 2) decoupling of electron transport from adenine nucleotide  transport and ATP production; 3) inhibition of ANT and ROS generation; 4) ROS stimulates  ER Ca2+ release; and 5) Ec also blocks Ca2+ influx, resulting in an ER stress response.	transcription
55470	3	335607	5	NULL	NULL	0	NULL	statement 2			results in					mitochondrial membrane		hyperpolarization of			NULL		0	NULL	NULL	NULL	gw70_molpharmacol_70_4_1424_s_269	16849592	1) Ec targets  complex III in the electron transport chain resulting in hyperpolarization of the  mitochondrial membrane; 2) decoupling of electron transport from adenine nucleotide  transport and ATP production; 3) inhibition of ANT and ROS generation; 4) ROS stimulates  ER Ca2+ release; and 5) Ec also blocks Ca2+ influx, resulting in an ER stress response.	transcription
56168	4	335607	5	NULL	NULL	0	NULL	electron transport			is decoupled from					adenine nucleotide transport					NULL		0	NULL	NULL	NULL	gw70_molpharmacol_70_4_1424_s_269	16849592	1) Ec targets  complex III in the electron transport chain resulting in hyperpolarization of the  mitochondrial membrane; 2) decoupling of electron transport from adenine nucleotide  transport and ATP production; 3) inhibition of ANT and ROS generation; 4) ROS stimulates  ER Ca2+ release; and 5) Ec also blocks Ca2+ influx, resulting in an ER stress response.	transcription
56169	5	335607	5	NULL	NULL	0	NULL	Ca2+ 			is release from					ER					NULL		0	NULL	NULL	NULL	gw70_molpharmacol_70_4_1424_s_269	16849592	1) Ec targets  complex III in the electron transport chain resulting in hyperpolarization of the  mitochondrial membrane; 2) decoupling of electron transport from adenine nucleotide  transport and ATP production; 3) inhibition of ANT and ROS generation; 4) ROS stimulates  ER Ca2+ release; and 5) Ec also blocks Ca2+ influx, resulting in an ER stress response.	transcription
56170	6	335607	5	NULL	NULL	0	NULL	ROS			stimulates					statement 5					NULL		0	NULL	NULL	NULL	gw70_molpharmacol_70_4_1424_s_269	16849592	1) Ec targets  complex III in the electron transport chain resulting in hyperpolarization of the  mitochondrial membrane; 2) decoupling of electron transport from adenine nucleotide  transport and ATP production; 3) inhibition of ANT and ROS generation; 4) ROS stimulates  ER Ca2+ release; and 5) Ec also blocks Ca2+ influx, resulting in an ER stress response.	transcription
56171	7	335607	5	NULL	NULL	0	NULL	Ec			block					Ca2+		influx of			NULL		0	NULL	NULL	NULL	gw70_molpharmacol_70_4_1424_s_269	16849592	1) Ec targets  complex III in the electron transport chain resulting in hyperpolarization of the  mitochondrial membrane; 2) decoupling of electron transport from adenine nucleotide  transport and ATP production; 3) inhibition of ANT and ROS generation; 4) ROS stimulates  ER Ca2+ release; and 5) Ec also blocks Ca2+ influx, resulting in an ER stress response.	transcription
56172	8	335607	5	NULL	NULL	0	NULL	statement 7			results in					ER stress response					NULL		0	NULL	NULL	NULL	gw70_molpharmacol_70_4_1424_s_269	16849592	1) Ec targets  complex III in the electron transport chain resulting in hyperpolarization of the  mitochondrial membrane; 2) decoupling of electron transport from adenine nucleotide  transport and ATP production; 3) inhibition of ANT and ROS generation; 4) ROS stimulates  ER Ca2+ release; and 5) Ec also blocks Ca2+ influx, resulting in an ER stress response.	transcription
60507	1	335607	7	NULL	NULL	0	NULL	Ec	Process		targets					complex III	GP				NULL		0	NULL	NULL	NULL	gw70_molpharmacol_70_4_1424_s_269	16849592	1) Ec targets  complex III in the electron transport chain resulting in hyperpolarization of the  mitochondrial membrane; 2) decoupling of electron transport from adenine nucleotide  transport and ATP production; 3) inhibition of ANT and ROS generation; 4) ROS stimulates  ER Ca2+ release; and 5) Ec also blocks Ca2+ influx, resulting in an ER stress response.	transcription
60508	2	335607	7	NULL	NULL	0	NULL	statement 1	Process		result in					mitochondrial membrane	CellComponent	hyperpolarization of			NULL		0	NULL	NULL	NULL	gw70_molpharmacol_70_4_1424_s_269	16849592	1) Ec targets  complex III in the electron transport chain resulting in hyperpolarization of the  mitochondrial membrane; 2) decoupling of electron transport from adenine nucleotide  transport and ATP production; 3) inhibition of ANT and ROS generation; 4) ROS stimulates  ER Ca2+ release; and 5) Ec also blocks Ca2+ influx, resulting in an ER stress response.	transcription
60509	3	335607	7	NULL	NULL	0	NULL	electron transport	Process		decoupled from					adenine nucleotide transport 	Process				NULL		0	NULL	NULL	NULL	gw70_molpharmacol_70_4_1424_s_269	16849592	1) Ec targets  complex III in the electron transport chain resulting in hyperpolarization of the  mitochondrial membrane; 2) decoupling of electron transport from adenine nucleotide  transport and ATP production; 3) inhibition of ANT and ROS generation; 4) ROS stimulates  ER Ca2+ release; and 5) Ec also blocks Ca2+ influx, resulting in an ER stress response.	transcription
60510	4	335607	7	NULL	NULL	0	NULL	electron transport	Process		decoupled from					ATP	Chemical	production of			NULL		0	NULL	NULL	NULL	gw70_molpharmacol_70_4_1424_s_269	16849592	1) Ec targets  complex III in the electron transport chain resulting in hyperpolarization of the  mitochondrial membrane; 2) decoupling of electron transport from adenine nucleotide  transport and ATP production; 3) inhibition of ANT and ROS generation; 4) ROS stimulates  ER Ca2+ release; and 5) Ec also blocks Ca2+ influx, resulting in an ER stress response.	transcription
60511	5	335607	7	NULL	NULL	0	NULL	statement 1	Process		leads to					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_molpharmacol_70_4_1424_s_269	16849592	1) Ec targets  complex III in the electron transport chain resulting in hyperpolarization of the  mitochondrial membrane; 2) decoupling of electron transport from adenine nucleotide  transport and ATP production; 3) inhibition of ANT and ROS generation; 4) ROS stimulates  ER Ca2+ release; and 5) Ec also blocks Ca2+ influx, resulting in an ER stress response.	transcription
60512	6	335607	7	NULL	NULL	0	NULL	statement 1	Process		leads to					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_molpharmacol_70_4_1424_s_269	16849592	1) Ec targets  complex III in the electron transport chain resulting in hyperpolarization of the  mitochondrial membrane; 2) decoupling of electron transport from adenine nucleotide  transport and ATP production; 3) inhibition of ANT and ROS generation; 4) ROS stimulates  ER Ca2+ release; and 5) Ec also blocks Ca2+ influx, resulting in an ER stress response.	transcription
60513	7	335607	7	NULL	NULL	0	NULL	statement 1	Process		leads to					ANT	Chemical	inhibition of			NULL		0	NULL	NULL	NULL	gw70_molpharmacol_70_4_1424_s_269	16849592	1) Ec targets  complex III in the electron transport chain resulting in hyperpolarization of the  mitochondrial membrane; 2) decoupling of electron transport from adenine nucleotide  transport and ATP production; 3) inhibition of ANT and ROS generation; 4) ROS stimulates  ER Ca2+ release; and 5) Ec also blocks Ca2+ influx, resulting in an ER stress response.	transcription
60514	8	335607	7	NULL	NULL	0	NULL	statement 1	Process		leads to					ROS	Chemical	generation of			NULL		0	NULL	NULL	NULL	gw70_molpharmacol_70_4_1424_s_269	16849592	1) Ec targets  complex III in the electron transport chain resulting in hyperpolarization of the  mitochondrial membrane; 2) decoupling of electron transport from adenine nucleotide  transport and ATP production; 3) inhibition of ANT and ROS generation; 4) ROS stimulates  ER Ca2+ release; and 5) Ec also blocks Ca2+ influx, resulting in an ER stress response.	transcription
60515	9	335607	7	NULL	NULL	0	NULL	ROS	Chemical		stimulate					Ca2+	Chemical	release of;;ER			NULL		0	NULL	NULL	NULL	gw70_molpharmacol_70_4_1424_s_269	16849592	1) Ec targets  complex III in the electron transport chain resulting in hyperpolarization of the  mitochondrial membrane; 2) decoupling of electron transport from adenine nucleotide  transport and ATP production; 3) inhibition of ANT and ROS generation; 4) ROS stimulates  ER Ca2+ release; and 5) Ec also blocks Ca2+ influx, resulting in an ER stress response.	transcription
60516	10	335607	7	NULL	NULL	0	NULL	Ec	Process		blocks					Ca2+ influx	Process				NULL		0	NULL	NULL	NULL	gw70_molpharmacol_70_4_1424_s_269	16849592	1) Ec targets  complex III in the electron transport chain resulting in hyperpolarization of the  mitochondrial membrane; 2) decoupling of electron transport from adenine nucleotide  transport and ATP production; 3) inhibition of ANT and ROS generation; 4) ROS stimulates  ER Ca2+ release; and 5) Ec also blocks Ca2+ influx, resulting in an ER stress response.	transcription
60517	11	335607	7	NULL	NULL	0	NULL	statement 10	Process		results in					stress response	Process				NULL		0	NULL	NULL	NULL	gw70_molpharmacol_70_4_1424_s_269	16849592	1) Ec targets  complex III in the electron transport chain resulting in hyperpolarization of the  mitochondrial membrane; 2) decoupling of electron transport from adenine nucleotide  transport and ATP production; 3) inhibition of ANT and ROS generation; 4) ROS stimulates  ER Ca2+ release; and 5) Ec also blocks Ca2+ influx, resulting in an ER stress response.	transcription
60518	12	335607	7	NULL	NULL	0	NULL	statement 1	Process		leads to					statement 9	Process				NULL		0	NULL	NULL	NULL	gw70_molpharmacol_70_4_1424_s_269	16849592	1) Ec targets  complex III in the electron transport chain resulting in hyperpolarization of the  mitochondrial membrane; 2) decoupling of electron transport from adenine nucleotide  transport and ATP production; 3) inhibition of ANT and ROS generation; 4) ROS stimulates  ER Ca2+ release; and 5) Ec also blocks Ca2+ influx, resulting in an ER stress response.	transcription
60519	1	335609	7	NULL	NULL	0	NULL	GDP	Chemical		inhibit					ATP synthase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_16_15534_s_207	15695816	Fig. 6 A shows that the nonphosphorylating oxygen consumption rates (state 4; expressed as nanomoles of oxygen atoms/min/mg of mitochondrial protein) of non-Dowex-treated BAT mitochondria from rats kept at room temperature in the presence of inhibitors of the adenine nucleotide carrier and ATP synthase is inhibited by addition of 1 mM GDP (from 175  plus-or-minus  6 to 128  plus-or-minus  5;  p = 0.0038).	transcription
60520	1	335612	7	NULL	NULL	0	NULL	2''-deoxyribose oligonucleotide	NucleicAcid		contain					adenine	Chemical				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6111_s_232	12167705	Because of the relative insensitivity of the 3H-based DNA  N-glycosylase release assay, DNA  N-glycosylase activity was measured by the more sensitive method, i.e., cleavage of a Tg residue-containing 2''-deoxyribose oligonucleotide which had been 5' end labeled with [gamma-32] and paired with a complementary 2''-deoxyribose oligonucleotide containing either an adenine or a guanine opposite Tg.	transcription
60521	2	335612	7	NULL	NULL	0	NULL	2''-deoxyribose oligonucleotide	NucleicAcid		contain					guanine	Chemical				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6111_s_232	12167705	Because of the relative insensitivity of the 3H-based DNA  N-glycosylase release assay, DNA  N-glycosylase activity was measured by the more sensitive method, i.e., cleavage of a Tg residue-containing 2''-deoxyribose oligonucleotide which had been 5' end labeled with [gamma-32] and paired with a complementary 2''-deoxyribose oligonucleotide containing either an adenine or a guanine opposite Tg.	transcription
60522	3	335612	7	NULL	NULL	0	NULL	Tg residue	Chemical		contain					2''-deoxyribose oligonucleotide	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6111_s_232	12167705	Because of the relative insensitivity of the 3H-based DNA  N-glycosylase release assay, DNA  N-glycosylase activity was measured by the more sensitive method, i.e., cleavage of a Tg residue-containing 2''-deoxyribose oligonucleotide which had been 5' end labeled with [gamma-32] and paired with a complementary 2''-deoxyribose oligonucleotide containing either an adenine or a guanine opposite Tg.	transcription
60523	4	335612	7	NULL	NULL	0	NULL	statement 3	Process		pair with					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6111_s_232	12167705	Because of the relative insensitivity of the 3H-based DNA  N-glycosylase release assay, DNA  N-glycosylase activity was measured by the more sensitive method, i.e., cleavage of a Tg residue-containing 2''-deoxyribose oligonucleotide which had been 5' end labeled with [gamma-32] and paired with a complementary 2''-deoxyribose oligonucleotide containing either an adenine or a guanine opposite Tg.	transcription
60524	5	335612	7	NULL	NULL	0	NULL	statement 3	Process		pair with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6111_s_232	12167705	Because of the relative insensitivity of the 3H-based DNA  N-glycosylase release assay, DNA  N-glycosylase activity was measured by the more sensitive method, i.e., cleavage of a Tg residue-containing 2''-deoxyribose oligonucleotide which had been 5' end labeled with [gamma-32] and paired with a complementary 2''-deoxyribose oligonucleotide containing either an adenine or a guanine opposite Tg.	transcription
60525	6	335612	7	NULL	NULL	0	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_17_6111_s_232	12167705	Because of the relative insensitivity of the 3H-based DNA  N-glycosylase release assay, DNA  N-glycosylase activity was measured by the more sensitive method, i.e., cleavage of a Tg residue-containing 2''-deoxyribose oligonucleotide which had been 5' end labeled with [gamma-32] and paired with a complementary 2''-deoxyribose oligonucleotide containing either an adenine or a guanine opposite Tg.	transcription
56173	1	335613	5	NULL	NULL	0	NULL	MutM			inhibit		severely			adenine		intrinsic rate of;;removal of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_25_22605_s_231	11960995	Conditions: DNA, 20 nM; active MutY, 5 nM; MutY alone ( closed circles), 480 nM MutM ( open circles), 480 nM Endo IV ( open triangles), 37  degrees C. Note that MutM severely inhibits the intrinsic rate of adenine removal, whereas similar concentrations of Endo IV only affect turnover.	transcription
60526	1	335613	7	NULL	NULL	0	NULL	 MutM	GP		inhibit		severely			adenine	Chemical	intrinsic rate of removal of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_25_22605_s_231	11960995	Conditions: DNA, 20 nM; active MutY, 5 nM; MutY alone ( closed circles), 480 nM MutM ( open circles), 480 nM Endo IV ( open triangles), 37  degrees C. Note that MutM severely inhibits the intrinsic rate of adenine removal, whereas similar concentrations of Endo IV only affect turnover.	transcription
60527	2	335613	7	NULL	NULL	0	NULL	Endo IV	GP		affect					adenine	Chemical	turnover of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_25_22605_s_231	11960995	Conditions: DNA, 20 nM; active MutY, 5 nM; MutY alone ( closed circles), 480 nM MutM ( open circles), 480 nM Endo IV ( open triangles), 37  degrees C. Note that MutM severely inhibits the intrinsic rate of adenine removal, whereas similar concentrations of Endo IV only affect turnover.	transcription
56185	2	335618	5	NULL	NULL	0	NULL	N6-adenine DNA Mtases M. TaqI		Thermus aquaticus	methylate					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_21_15066_s_36	10329711	In this publication we show that the  N6-adenine DNA Mtases M. TaqI from  Thermus aquaticus ( 23,  24) and M. CviBIII from the  Chlorella virus NC-1A ( 25), which both methylate adenine within the double-stranded 5''-TCGA-3' DNA sequence, give high photo-cross-linking yields with duplex ODNs containing 5-iodouracil at the target position (Scheme  1).	transcription
56186	1	335618	5	NULL	NULL	0	NULL	adenine			is present within					DNA sequence		double-stranded		5''-TCGA-3' 	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_15066_s_36	10329711	In this publication we show that the  N6-adenine DNA Mtases M. TaqI from  Thermus aquaticus ( 23,  24) and M. CviBIII from the  Chlorella virus NC-1A ( 25), which both methylate adenine within the double-stranded 5''-TCGA-3' DNA sequence, give high photo-cross-linking yields with duplex ODNs containing 5-iodouracil at the target position (Scheme  1).	transcription
56187	3	335618	5	NULL	NULL	0	NULL	M. CviBIII		Chlorella virus NC-1A	methylate					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_21_15066_s_36	10329711	In this publication we show that the  N6-adenine DNA Mtases M. TaqI from  Thermus aquaticus ( 23,  24) and M. CviBIII from the  Chlorella virus NC-1A ( 25), which both methylate adenine within the double-stranded 5''-TCGA-3' DNA sequence, give high photo-cross-linking yields with duplex ODNs containing 5-iodouracil at the target position (Scheme  1).	transcription
60528	1	335618	7	NULL	NULL	0	NULL	M. TaqI	GP	Thermus aquaticus	methylate					adenine 	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_21_15066_s_36	10329711	In this publication we show that the  N6-adenine DNA Mtases M. TaqI from  Thermus aquaticus ( 23,  24) and M. CviBIII from the  Chlorella virus NC-1A ( 25), which both methylate adenine within the double-stranded 5''-TCGA-3' DNA sequence, give high photo-cross-linking yields with duplex ODNs containing 5-iodouracil at the target position (Scheme  1).	transcription
60529	2	335618	7	NULL	NULL	0	NULL	statement 1	Process		occur within							double-stranded		5''-TCGA-3' DNA sequence	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_21_15066_s_36	10329711	In this publication we show that the  N6-adenine DNA Mtases M. TaqI from  Thermus aquaticus ( 23,  24) and M. CviBIII from the  Chlorella virus NC-1A ( 25), which both methylate adenine within the double-stranded 5''-TCGA-3' DNA sequence, give high photo-cross-linking yields with duplex ODNs containing 5-iodouracil at the target position (Scheme  1).	transcription
60530	3	335618	7	NULL	NULL	0	NULL	M. CviBIII	GP	Chlorella virus NC-1A	methylate					adenine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_21_15066_s_36	10329711	In this publication we show that the  N6-adenine DNA Mtases M. TaqI from  Thermus aquaticus ( 23,  24) and M. CviBIII from the  Chlorella virus NC-1A ( 25), which both methylate adenine within the double-stranded 5''-TCGA-3' DNA sequence, give high photo-cross-linking yields with duplex ODNs containing 5-iodouracil at the target position (Scheme  1).	transcription
60531	4	335618	7	NULL	NULL	0	NULL	statement 3	Process		occur within							double-stranded		5''-TCGA-3' DNA sequence	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_21_15066_s_36	10329711	In this publication we show that the  N6-adenine DNA Mtases M. TaqI from  Thermus aquaticus ( 23,  24) and M. CviBIII from the  Chlorella virus NC-1A ( 25), which both methylate adenine within the double-stranded 5''-TCGA-3' DNA sequence, give high photo-cross-linking yields with duplex ODNs containing 5-iodouracil at the target position (Scheme  1).	transcription
60532	5	335618	7	NULL	NULL	0	NULL	M. TaqI	GP	Thermus aquaticus	is a type of					N6-adenine DNA Mtases	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_21_15066_s_36	10329711	In this publication we show that the  N6-adenine DNA Mtases M. TaqI from  Thermus aquaticus ( 23,  24) and M. CviBIII from the  Chlorella virus NC-1A ( 25), which both methylate adenine within the double-stranded 5''-TCGA-3' DNA sequence, give high photo-cross-linking yields with duplex ODNs containing 5-iodouracil at the target position (Scheme  1).	transcription
60533	6	335618	7	NULL	NULL	0	NULL	M. CviBIII	GP	Chlorella virus NC-1A	is a type of					N6-adenine DNA Mtases	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_21_15066_s_36	10329711	In this publication we show that the  N6-adenine DNA Mtases M. TaqI from  Thermus aquaticus ( 23,  24) and M. CviBIII from the  Chlorella virus NC-1A ( 25), which both methylate adenine within the double-stranded 5''-TCGA-3' DNA sequence, give high photo-cross-linking yields with duplex ODNs containing 5-iodouracil at the target position (Scheme  1).	transcription
56188	1	335619	5	NULL	NULL	0	NULL	apoptosis			is mediated by					TNF-alpha					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
56189	2	335619	5	NULL	NULL	0	NULL	ceramides			is involved in					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
56190	3	335619	5	NULL	NULL	0	NULL	protein-phosphatase			is activated by					ceramide					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
56191	4	335619	5	NULL	NULL	0	NULL	statement 3			is involved in					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
56192	5	335619	5	NULL	NULL	0	NULL	protein kinase II			is dependent on					calmodulin					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
56193	6	335619	5	NULL	NULL	0	NULL	statement 5			is involved in					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
56194	7	335619	5	NULL	NULL	0	NULL	nicotinamide adenine dinucleotide			is involved in					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
56195	8	335619	5	NULL	NULL	0	NULL	P24			is involved in					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
56196	9	335619	5	NULL	NULL	0	NULL	P21/WAF-1			is involved in					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
56197	10	335619	5	NULL	NULL	0	NULL	mitochondrial respiratory insufficiency			is involved in					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
56198	11	335619	5	NULL	NULL	0	NULL	NFkB			is involved in					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
56199	12	335619	5	NULL	NULL	0	NULL	phospholipase D			is involved in					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
60534	1	335619	7	NULL	NULL	0	NULL	TNF-alpha	GP		mediate					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
60535	2	335619	7	NULL	NULL	0	NULL	ceramides 	Chemical		is involved in					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
60536	3	335619	7	NULL	NULL	0	NULL	ceramide	Chemical		activate					protein-phosphatase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
60537	4	335619	7	NULL	NULL	0	NULL	statement 3	Process		is involved in					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
60538	5	335619	7	NULL	NULL	0	NULL	calmodulin-dependent protein kinase II 	GP		is involved in					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
60539	6	335619	7	NULL	NULL	0	NULL	 nicotinamide adenine dinucleotide	Chemical		is involved in					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
60540	7	335619	7	NULL	NULL	0	NULL	P24	GP		is involved in					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
60541	8	335619	7	NULL	NULL	0	NULL	P21/WAF-1	GP		is involved in					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
60542	9	335619	7	NULL	NULL	0	NULL	mitochondrial respiratory insufficiency 	Process		is involved in					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
60543	10	335619	7	NULL	NULL	0	NULL	NFkB	GP		is involved in					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
60544	11	335619	7	NULL	NULL	0	NULL	phospholipase D	GP		is involved in					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
60545	12	335619	7	NULL	NULL	0	NULL	ceramides	Chemical		is a type of					signaling factor	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
60546	13	335619	7	NULL	NULL	0	NULL	ceramide-activated protein-phosphatase	GP		is a type of					signaling factor	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
60547	14	335619	7	NULL	NULL	0	NULL	calmodulin-dependent protein kinase II	GP		is a type of					signaling factor	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
60548	15	335619	7	NULL	NULL	0	NULL	nicotinamide adenine dinucleotide	Chemical		is a type of					signaling factor	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
60549	16	335619	7	NULL	NULL	0	NULL	P24	GP		is a type of					signaling factor	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
60550	17	335619	7	NULL	NULL	0	NULL	P21/WAF-1	GP		is a type of					signaling factor	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
60551	18	335619	7	NULL	NULL	0	NULL	mitochondrial respiratory insufficiency	Process		is a type of					signaling factor	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
60552	19	335619	7	NULL	NULL	0	NULL	NFkB	GP		is a type of					signaling factor	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
60553	20	335619	7	NULL	NULL	0	NULL	phospholipase D	GP		is a type of					signaling factor	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23526_s_11	10438532	Numerous signaling factors have been reported to be involved in the apoptosis process mediated by TNF-alpha, including ceramides and ceramide-activated protein-phosphatase ( 3), calmodulin-dependent protein kinase II ( 4), nicotinamide adenine dinucleotide and P24 ( 5), P21/WAF-1 ( 6), mitochondrial respiratory insufficiency ( 7), NFkB ( 8), and phospholipase D ( 9).	transcription
56485	1	335623	5	NULL	NULL	0	NULL	PDGF			induces					DNA		synthesis of			NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
58494	2	335623	5	NULL	NULL	0	NULL	antisense oligonucleotides to A(2B) receptor			increases					DNA synthesis		basal			NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
58495	3	335623	5	NULL	NULL	0	NULL	antisense oligonucleotides to A(2B) receptor			increases					statement 1					NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
58496	4	335623	5	NULL	NULL	0	NULL	sense oligonucleotides to A(2B) receptor			does not increase					statement 1					NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
58497	5	335623	5	NULL	NULL	0	NULL	sense oligonucleotides to A(2B) receptor			does not increase					DNA synthesis		basal			NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
58498	6	335623	5	NULL	NULL	0	NULL	scrambled oligonucleotides to A(2B) receptor			does not increase					statement 1					NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
58499	7	335623	5	NULL	NULL	0	NULL	scrambled oligonucleotides to A(2B) receptor			does not increase					DNA synthesis		basal			NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
58500	8	335623	5	NULL	NULL	0	NULL	antisense oligonucleotides to A(2B) receptor			increases					cell proliferation					NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
58501	9	335623	5	NULL	NULL	0	NULL	sense oligonucleotides to A(2B) receptor			does not increase					cell proliferation					NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
58502	10	335623	5	NULL	NULL	0	NULL	scrambled oligonucleotides to A(2B) receptor			does not increase					cell proliferation					NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
58503	11	335623	5	NULL	NULL	0	NULL	antisense oligonucleotides to A(2B) receptor			increases					collagen		synthesis of			NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
58504	12	335623	5	NULL	NULL	0	NULL	sense oligonucleotides to A(2B) receptor			does not increase					collagen		synthesis of			NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
58505	13	335623	5	NULL	NULL	0	NULL	antisense oligonucleotides to A(2B) receptor			abolishes					2-chloroadenosine		growth-inhibitory effects of 			NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
58506	14	335623	5	NULL	NULL	0	NULL	sense oligonucleotides to A(2B) receptor			does not abolish					2-chloroadenosine		growth-inhibitory effects of 			NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
58507	15	335623	5	NULL	NULL	0	NULL	scrambled oligonucleotides to A(2B) receptor			does not abolish					2-chloroadenosine		growth-inhibitory effects of			NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
58508	16	335623	5	NULL	NULL	0	NULL	antisense oligonucleotides to A(2B) receptor			abolishes					5''-N-MECA		growth-inhibitory effects of			NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
58509	17	335623	5	NULL	NULL	0	NULL	sense oligonucleotides to A(2B) receptor			does not abolish					5''-N-MECA		growth-inhibitory effects of			NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
58510	18	335623	5	NULL	NULL	0	NULL	scrambled oligonucleotides to A(2B) receptor			does not abolish					5''-N-MECA		growth-inhibitory effects of			NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
58511	19	335623	5	NULL	NULL	0	NULL	antisense oligonucleotides to A(2B) receptor			abolishes					erythro-9-(2-hydroxy-3-nonyl)adenine		growth-inhibitory effects of			NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
58512	20	335623	5	NULL	NULL	0	NULL	sense oligonucleotides to A(2B) receptor			does not abolish					erythro-9-(2-hydroxy-3-nonyl)adenine		growth-inhibitory effects of			NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
58513	21	335623	5	NULL	NULL	0	NULL	scrambled oligonucleotides to A(2B) receptor			does not abolish					erythro-9-(2-hydroxy-3-nonyl)adenine		growth-inhibitory effects of			NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
58514	22	335623	5	NULL	NULL	0	NULL	antisense oligonucleotides to A(2B) receptor			abolishes					iodotubercidin		growth-inhibitory effects of			NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
58515	23	335623	5	NULL	NULL	0	NULL	sense oligonucleotides to A(2B) receptor			does not abolish					iodotubercidin		growth-inhibitory effects of			NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
58516	24	335623	5	NULL	NULL	0	NULL	scrambled oligonucleotides to A(2B) receptor			does not abolish					iodotubercidin		growth-inhibitory effects of			NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
58517	25	335623	5	NULL	NULL	0	NULL	iodotubercidin			is an inhibitor of					adenosine kinase					NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
58518	26	335623	5	NULL	NULL	0	NULL	erythro-9-(2-hydroxy-3-nonyl)adenine			is an inhibitor of					adenosine deaminase					NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60555	1	335623	7	NULL	NULL	0	NULL	PDGF	GP		induce					DNA 	NucleicAcid	synthesis of			NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60556	2	335623	7	NULL	NULL	0	NULL	A(2B) receptor	GP	antisense oligonucleotides to 	increase					DNA	NucleicAcid	basal synthesis of			NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60557	3	335623	7	NULL	NULL	0	NULL	A(2B) receptor	GP	antisense oligonucleotides to 	increase					statement 1	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60558	4	335623	7	NULL	NULL	0	NULL	A(2B) receptor	GP	antisense oligonucleotides to 	increase					cell proliferation	Process				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60559	5	335623	7	NULL	NULL	0	NULL	A(2B) receptor	GP	antisense oligonucleotides to 	increase					collagen	GP	synthesis of			NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60560	6	335623	7	NULL	NULL	0	NULL	2-chloroadenosine	Chemical		inhibit					growth	Process				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60561	7	335623	7	NULL	NULL	0	NULL	A(2B) receptor	GP	antisense oligonucleotides to 	abolish					statement 6	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60562	9	335623	7	NULL	NULL	0	NULL	A(2B) receptor	GP	antisense oligonucleotides to 	abolish					statement 8	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60563	11	335623	7	NULL	NULL	0	NULL	A(2B) receptor	GP	antisense oligonucleotides to 	abolish					statement 10	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60564	8	335623	7	NULL	NULL	0	NULL	 5''-N-MECA	Chemical		inhibit					growth	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60565	10	335623	7	NULL	NULL	0	NULL	erythro-9-(2-hydroxy-3-nonyl)adenine	Chemical		inhibit					growth	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60566	12	335623	7	NULL	NULL	0	NULL	 5''-N-MECA	Chemical		is an inhibitor of					adenosine deaminase	GP				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60567	13	335623	7	NULL	NULL	0	NULL	erythro-9-(2-hydroxy-3-nonyl)adenine	Chemical		is an inhibitor of					adenosine deaminase	GP				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60568	14	335623	7	NULL	NULL	0	NULL	iodotubercidin	Chemical		inhibit					growth	Process				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60569	15	335623	7	NULL	NULL	0	NULL	A(2B) receptor	GP	 antisense oligonucleotide to	abolish					statement 14	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60570	16	335623	7	NULL	NULL	0	NULL	iodotubercidin	Chemical		is an inhibitor of					adenosine kinase	GP				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60574	17	335623	7	NULL	NULL	0	NULL	A(2B) receptor	GP	sense oligonucleotide to	does not increase					DNA	NucleicAcid	synthesis of basal			NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60575	18	335623	7	NULL	NULL	0	NULL	A(2B) receptor	GP	sense oligonucleotide to	does not increase					statement 1	Process				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60576	19	335623	7	NULL	NULL	0	NULL	A(2B) receptor	GP	sense oligonucleotide to	does not increase					cell proliferation	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60577	20	335623	7	NULL	NULL	0	NULL	A(2B) receptor	GP	sense oligonucleotide to	does not increase					collagen	GP	synthesis of			NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60578	21	335623	7	NULL	NULL	0	NULL	A(2B) receptor	GP	sense oligonucleotide to	does not abolish					statement 6	Process				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60579	22	335623	7	NULL	NULL	0	NULL	A(2B) receptor	GP	sense oligonucleotide to	does not abolish					statement 8	Process				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60580	23	335623	7	NULL	NULL	0	NULL	A(2B) receptor	GP	sense oligonucleotide to	does not abolish					statement 10	Process				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60581	24	335623	7	NULL	NULL	0	NULL	A(2B) receptor	GP	sense oligonucleotide to	does not abolish					statement 14	Process				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60582	25	335623	7	NULL	NULL	0	NULL	A(2B) receptor	GP	scrambled oligonucleotide to	does not increase					DNA	NucleicAcid	synthesis of basal			NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60583	26	335623	7	NULL	NULL	0	NULL	A(2B) receptor	GP	scrambled oligonucleotide to	does not increase					statement 1	Process				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60584	27	335623	7	NULL	NULL	0	NULL	A(2B) receptor	GP	scrambled oligonucleotide to	does not increase					cell proliferation	Process				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60585	28	335623	7	NULL	NULL	0	NULL	A(2B) receptor	GP	scrambled oligonucleotide to	does not increase					collagen	GP	synthesis of			NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60586	29	335623	7	NULL	NULL	0	NULL	A(2B) receptor	GP	scrambled oligonucleotide to	does not abolish					statement 6	Process				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60587	30	335623	7	NULL	NULL	0	NULL	A(2B) receptor	GP	scrambled oligonucleotide to	does not abolish					statement 8	Process				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60588	31	335623	7	NULL	NULL	0	NULL	A(2B) receptor	GP	scrambled oligonucleotide to	does not abolish					statement 10	Process				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
60589	32	335623	7	NULL	NULL	0	NULL	A(2B) receptor	GP	scrambled oligonucleotide to	does not abolish					statement 14	Process				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_hypertension_46_3_16103269_s_4	16103269	Antisense, but not sense or scrambled,  oligonucleotides to the A(2B) receptor increased both basal and PDGF-induced  DNA synthesis, cell proliferation, and collagen synthesis, and the growth-inhibitory  effects of 2-chloroadenosine, 5''-N-MECA, and erythro-9-(2-hydroxy-3-nonyl)adenine  (inhibitor of adenosine deaminase) plus iodotubercidin (inhibitor of adenosine  kinase) were abolished by antisense, but not scrambled or sense, oligonucleotides  to the A(2B) receptor.	transcription
56486	1	335626	5	NULL	NULL	0	NULL	BH3 only proteins			induces		autonomously			cytochrome c		release of			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
56487	2	335626	5	NULL	NULL	0	NULL	BCL-2 family			does not participate in					statement 1					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
56488	3	335626	5	NULL	NULL	0	NULL	mitochondrial proteins		intrinsic	does not participate in					statement 1					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
56489	4	335626	5	NULL	NULL	0	NULL	cardiolipin			is required for					statement 1					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
56490	5	335626	5	NULL	NULL	0	NULL	cardiolipin			is a type of					negatively charged lipids					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
56491	6	335626	5	NULL	NULL	0	NULL	BAX			is a type of					proapoptotic protein					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
56492	7	335626	5	NULL	NULL	0	NULL	BAK			is a type of					proapoptotic protein					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
56493	8	335626	5	NULL	NULL	0	NULL	BAX		activated	mediates					cytochrome c		release of			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
56494	9	335626	5	NULL	NULL	0	NULL	BAK		activated	mediates					cytochrome c		release of			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
56495	10	335626	5	NULL	NULL	0	NULL	ANT			is					adenine nucleotide exchanger					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
56496	11	335626	5	NULL	NULL	0	NULL	VDAC			is					voltage dependent anion channel					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
60590	1	335626	7	NULL	NULL	0	NULL	BH3 only proteins	GP		induce		autonomously			cytochrome c	GP	release of			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
60591	2	335626	7	NULL	NULL	0	NULL	statement 1	Process		does not involve					BCL-2 family	GP				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
60592	3	335626	7	NULL	NULL	0	NULL	statement 1	Process		does not involve					intrinsic mitochondrial proteins	GP				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
60593	4	335626	7	NULL	NULL	0	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
60594	5	335626	7	NULL	NULL	0	NULL	statement 1	Process		require					cardiolipin	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
60595	6	335626	7	NULL	NULL	0	NULL	cardiolipin	Chemical		is a type of					negatively charged lipid	Chemical				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
60596	7	335626	7	NULL	NULL	0	NULL	BH3 only proteins	GP		interact with					antiapoptotic BCL-2 family members	GP				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
60597	8	335626	7	NULL	NULL	0	NULL	BH3 only proteins	GP		inhibit					antiapoptotic BCL-2 family members	GP				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
60598	9	335626	7	NULL	NULL	0	NULL	BH3 only proteins	GP		activate					proapoptotic BAX	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
60599	10	335626	7	NULL	NULL	0	NULL	BH3 only proteins	GP		activate					proapoptotic BAK	GP				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
60600	11	335626	7	NULL	NULL	0	NULL	statement 9	Process		mediate					cytochrome	GP	release of			NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
60601	12	335626	7	NULL	NULL	0	NULL	statement 10	Process		mediate					cytochrome	GP	release of			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
60602	13	335626	7	NULL	NULL	0	NULL	BH3 only proteins	GP		interact with					ANT	GP				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
60603	14	335626	7	NULL	NULL	0	NULL	BH3 only proteins	GP		interact with					VDAC	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
60604	15	335626	7	NULL	NULL	0	NULL	statement 13	Process		induce					mitochondrial dysfunction	CellComponent				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
60605	16	335626	7	NULL	NULL	0	NULL	statement 14	Process		induce					mitochondrial dysfunction	CellComponent				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
60606	17	335626	7	NULL	NULL	0	NULL	statement 13	Process		induce					cytochrome c	GP	release of			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
60607	18	335626	7	NULL	NULL	0	NULL	statement 14	Process		induce					cytochrome c	GP	release of			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
60608	19	335626	7	NULL	NULL	0	NULL	statement 13	Process		is an alternative to					statement 14	Process				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
60609	20	335626	7	NULL	NULL	0	NULL	ANT	GP		is					adenine nucleotide exchanger 	GP				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
60610	21	335626	7	NULL	NULL	0	NULL	VDAC	GP		is					voltage dependent anion channel 	GP				NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
60611	22	335626	7	NULL	NULL	0	NULL	ANT	GP		is a type of					 intrinsic mitochondrial proteins 	GP				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
60612	23	335626	7	NULL	NULL	0	NULL	VDAC	GP		is a type of					intrinsic mitochondrial proteins	GP				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_304_3_437_s_7	12729577	At least four main different models have been put  forth: (i) BH3 only proteins autonomously induce cytochrome  c release, without the participation of BCL-2 family or intrinsic mitochondrial proteins  but with a marked requirement for negatively charged lipids such as cardiolipin [  15 and   16]; (ii) they interact and inhibit antiapoptotic BCL-2 family members [  17,   18,   19,   20 and   21]; (iii) they activate the multidomain proapoptotic BAX and BAK to mediate cytochrome   c release [ 5,   22 and   23]; (iv) they interact with intrinsic mitochondrial proteins such as the adenine nucleotide  exchanger (ANT) or the voltage dependent anion channel (VDAC) to induce mitochondrial  dysfunction and cytochrome  c release [  24 and   25].	transcription
56499	3	335629	5	NULL	NULL	0	NULL	long chain fatty acyl-CoAs			regulates		may			metabolism		intermediary			NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
56500	4	335629	5	NULL	NULL	0	NULL	glucokinase		modulation of;;activity of	leads to					statement 3					NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
58519	1	335629	5	NULL	NULL	0	NULL	free acids		CoA-thioesterification of;;xenobiotic	produces		endogenously			acyl-CoAs		xenobiotic			NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
58520	2	335629	5	NULL	NULL	0	NULL	statement 1			is dependent on					ATP					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
58521	5	335629	5	NULL	NULL	0	NULL	pyruvate dehydrogenase		modulation of;;activity of	leads to					statement 3					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
58522	6	335629	5	NULL	NULL	0	NULL	acetyl-CoA carboxylase		modulation of;;activity of	leads to					statement 3					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
58523	7	335629	5	NULL	NULL	0	NULL	delta9-desaturase		modulation of;;activity of	leads to					statement 3					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
58524	8	335629	5	NULL	NULL	0	NULL	protein kinase C		modulation of;;activity of	leads to					statement 3					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
58525	9	335629	5	NULL	NULL	0	NULL	adenine nucleotide translocase		modulation of;;activity of;;mitochondrial	leads to					statement 3					NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
58526	10	335629	5	NULL	NULL	0	NULL	citrate transporter		modulation of;;activity of;;mitochondrial	leads to					statement 3					NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
58527	11	335629	5	NULL	NULL	0	NULL	Na/K ATPase		modulation of;;activity of	leads to					statement 3					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
58528	12	335629	5	NULL	NULL	0	NULL	ATP-sensitive K-channels		modulation of;;activity of	leads to					statement 3					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
58529	13	335629	5	NULL	NULL	0	NULL	Ca-ATPase		modulation of;;activity of;;endoplasmic reticulum	leads to					statement 3					NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
58530	14	335629	5	NULL	NULL	0	NULL	transcription factors		modulation of;;activity of	leads to					statement 3					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
58531	15	335629	5	NULL	NULL	0	NULL	acyl-CoAs		xenobiotic	regulates		may			metabolism		intermediary			NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
58532	16	335629	5	NULL	NULL	0	NULL	glucokinase		modulation of;;activity of	leads to					statement 15					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
58533	17	335629	5	NULL	NULL	0	NULL	pyruvate dehydrogenase		modulation of;;activity of	leads to					statement 15					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
58534	18	335629	5	NULL	NULL	0	NULL	acetyl-CoA carboxylase		modulation of;;activity of	leads to					statement 15					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
58535	19	335629	5	NULL	NULL	0	NULL	delta9-desaturase		modulation of;;activity of	leads to					statement 15					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
58536	20	335629	5	NULL	NULL	0	NULL	protein kinase C		modulation of;;activity of	leads to					statement 15					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
58537	21	335629	5	NULL	NULL	0	NULL	adenine nucleotide translocase		modulation of;;activity of;;mitochondrial	leads to					statement 15					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
58538	22	335629	5	NULL	NULL	0	NULL	citrate transporter		modulation of;;activity of;;mitochondrial	leads to					statement 15					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
58539	23	335629	5	NULL	NULL	0	NULL	Na/K ATPase		modulation of;;activity of	leads to					statement 15					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
58540	24	335629	5	NULL	NULL	0	NULL	ATP-sensitive K-channels		modulation of;;activity of	leads to					statement 15					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
58541	25	335629	5	NULL	NULL	0	NULL	Ca-ATPase		modulation of;;activity of;;endoplasmic reticulum	leads to					statement 15					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
58542	26	335629	5	NULL	NULL	0	NULL	transcription factors		modulation of;;activity of	leads to					statement 15					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
58543	27	335629	5	NULL	NULL	0	NULL	adenine nucleotide translocase		mitochondrial	is a type of					transporter					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
58544	28	335629	5	NULL	NULL	0	NULL	citrate transporter		mitochondrial	is a type of					transporter					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
58545	29	335629	5	NULL	NULL	0	NULL	Na/K ATPase			is a type of					transporter					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
58546	30	335629	5	NULL	NULL	0	NULL	ATP-sensitive K-channels			is a type of					ion channel					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
58547	31	335629	5	NULL	NULL	0	NULL	Ca-ATPase		endoplasmic reticulum	is a type of					ion channel					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60613	1	335629	7	NULL	NULL	0	NULL	long chain fatty acyl-CoA 	Chemical		regulate		may			intermediary metabolism	Process				NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60614	2	335629	7	NULL	NULL	0	NULL	statement 1	Process		occur by					glucokinase	GP	modulating			NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60615	3	335629	7	NULL	NULL	0	NULL	statement 1	Process		occur by					pyruvate dehydrogenase	GP	modulating			NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60616	4	335629	7	NULL	NULL	0	NULL	statement 1	Process		occur by					acetyl-CoA carboxylase	GP	modulating			NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60617	5	335629	7	NULL	NULL	0	NULL	statement 1	Process		occur by					delta9-desaturase	GP	modulating			NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60618	6	335629	7	NULL	NULL	0	NULL	statement 1	Process		occur by					protein kinase C	GP	modulating			NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60619	7	335629	7	NULL	NULL	0	NULL	statement 1	Process		occur by					mitochondrial adenine nucleotide translocase	GP	modulating			NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60620	8	335629	7	NULL	NULL	0	NULL	statement 1	Process		occur by					mitochondrial citrate transporter	GP	modulating			NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60621	9	335629	7	NULL	NULL	0	NULL	statement 1	Process		occur by					Na/K ATPase	GP	modulating			NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60622	10	335629	7	NULL	NULL	0	NULL	statement 1	Process		occur by					ATP-sensitive K-channels	CellComponent	modulating			NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60623	11	335629	7	NULL	NULL	0	NULL	statement 1	Process		occur by					endoplasmic reticulum Ca-ATPase	GP	modulating			NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60624	12	335629	7	NULL	NULL	0	NULL	statement 1	Process		occur by					transcription factors	GP	modulating			NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60625	13	335629	7	NULL	NULL	0	NULL	xenobiotic acyl-CoAs	Chemical		produced by					xenobiotic free acids	Chemical				NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60626	14	335629	7	NULL	NULL	0	NULL	statement 13	Process		produced by		endogenously			ATP-dependent CoA-thioesterification	Process				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60627	15	335629	7	NULL	NULL	0	NULL	statement 13	Process		regulate		may			intermediary metabolism	Process				NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60628	16	335629	7	NULL	NULL	0	NULL	statement 15	Process		occur by					glucokinase	GP	modulating			NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60629	17	335629	7	NULL	NULL	0	NULL	statement 15	Process		occur by					pyruvate dehydrogenase	GP	modulating			NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60630	18	335629	7	NULL	NULL	0	NULL	statement 15	Process		occur by					acetyl-CoA carboxylase	GP	modulating			NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60631	19	335629	7	NULL	NULL	0	NULL	statement 15	Process		occur by					delta9-desaturase	GP	modulating			NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60632	20	335629	7	NULL	NULL	0	NULL	statement 15	Process		occur by					protein kinase C	GP	modulating			NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60633	21	335629	7	NULL	NULL	0	NULL	statement 15	Process		occur by					mitochondrial adenine nucleotide translocase	GP	modulating			NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60634	22	335629	7	NULL	NULL	0	NULL	statement 15	Process		occur by					mitochondrial citrate transporter	GP	modulating			NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60635	23	335629	7	NULL	NULL	0	NULL	statement 15	Process		occur by					 Na/K ATPase	GP	modulating			NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60636	24	335629	7	NULL	NULL	0	NULL	statement 15	Process		occur by					ATP-sensitive K-channels	CellComponent	modulating			NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60637	25	335629	7	NULL	NULL	0	NULL	statement 15	Process		occur by					endoplasmic reticulum Ca-ATPase	GP	modulating			NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60638	26	335629	7	NULL	NULL	0	NULL	statement 15	Process		occur by					transcription factors	GP	modulating			NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60639	27	335629	7	NULL	NULL	0	NULL	mitochondrial adenine nucleotide translocase	GP		is a type of					transporter	GP				NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60640	28	335629	7	NULL	NULL	0	NULL	mitochondrial citrate transporter	GP		is a type of					transporter	GP				NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60641	29	335629	7	NULL	NULL	0	NULL	Na/K ATPase	GP		is a type of					transporter	GP				NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60642	30	335629	7	NULL	NULL	0	NULL	ATP-sensitive K-channels	CellComponent		is a type of					ion channel	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
60643	31	335629	7	NULL	NULL	0	NULL	endoplasmic reticulum Ca-ATPase	GP		is a type of					ion channel	GP				NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_7_1125_s_12	12091497	In addition to their substrate role, long chain fatty acyl-CoAs, as well as xenobiotic acyl-CoAs endogenously produced by ATP-dependent CoA-thioesterification of the respective xenobiotic free acids ( 1), may regulate intermediary metabolism by modulating the activity of enzymes (e.g., glucokinase, pyruvate dehydrogenase, acetyl-CoA carboxylase, delta9-desaturase, protein kinase C), transporters (e.g., mitochondrial adenine nucleotide translocase, mitochondrial citrate transporter, Na/K ATPase), ion channels (e.g., ATP-sensitive K-channels, endoplasmic reticulum Ca-ATPase) ( 2 -  4), or transcription factors ( 5 -  9).	transcription
56234	1	335630	5	NULL	NULL	0	NULL	NOS isozymes			is activated by					calcium		intracellular 			NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
56235	2	335630	5	NULL	NULL	0	NULL	iNOS			bind			NOSox		heme					NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
56236	3	335630	5	NULL	NULL	0	NULL	NOSox			is					NH2-terminal catalytic oxygenase domain					NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
56237	4	335630	5	NULL	NULL	0	NULL	iNOS			resides in			NOSox		iNOS			residues 1 to 498		NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
56238	5	335630	5	NULL	NULL	0	NULL	heme			is					iron protoporphyrin IX					NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
56239	6	335630	5	NULL	NULL	0	NULL	iNOS			bind			NOSox		tetrahydrobiopterin					NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
56240	7	335630	5	NULL	NULL	0	NULL	tetrahydrobiopterin			is					H4B					NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
56241	8	335630	5	NULL	NULL	0	NULL	iNOS			bind			NOSox		L-Arg					NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
56242	9	335630	5	NULL	NULL	0	NULL	L-Arg			is a type of					substrate					NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
56243	10	335630	5	NULL	NULL	0	NULL	iNOS			bind			NOSred		FMN					NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
56244	11	335630	5	NULL	NULL	0	NULL	FMN			is					flavin mononucleotide 					NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
56245	12	335630	5	NULL	NULL	0	NULL	NOSred			is					COOH-terminal reductase domain					NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
56246	13	335630	5	NULL	NULL	0	NULL	iNOS			resides in			NOSred		iNOS			residues 531 to 1144		NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
56247	14	335630	5	NULL	NULL	0	NULL	iNOS			bind			NOSred		FAD					NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
56248	15	335630	5	NULL	NULL	0	NULL	FAD			is					flavin adenine dinucleotide					NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
56249	16	335630	5	NULL	NULL	0	NULL	iNOS			bind			NOSred		NADPH					NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
56250	17	335630	5	NULL	NULL	0	NULL	iNOS			communicates with		electronic	NOSox		iNOS			NOSred		NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
56251	18	335630	5	NULL	NULL	0	NULL	iNOS			resides in			calmodulin-binding region		iNOS			residues 499 to 530		NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
56252	19	335630	5	NULL	NULL	0	NULL	iNOS			regulates			calmodulin-binding region		statement 17					NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
60644	1	335630	7	NULL	NULL	0	NULL	iNOS	GP		bind			NOSox, residues 1 to 498		iron protoporphyrin IX	Chemical				NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
60645	2	335630	7	NULL	NULL	0	NULL	i NOS	GP		bind			NOSox, residues 1 to 498		H4B	Chemical				NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
60646	3	335630	7	NULL	NULL	0	NULL	iNOS	GP		bind			NOSox, residues 1 to 498		L-Arg	AminoAcid				NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
60647	4	335630	7	NULL	NULL	0	NULL	iNOS			is a type of			NOSox, residues 1 to 498					NH2-terminal catalytic oxygenase domain		NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
60648	5	335630	7	NULL	NULL	0	NULL	H4B	Chemical		is					tetrahydrobiopterin	Chemical				NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
60649	6	335630	7	NULL	NULL	0	NULL	iNOS	GP		bind			NOSred, residues 531 to 1144		FMN	Chemical				NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
60650	7	335630	7	NULL	NULL	0	NULL	iNOS			bind			NOSred, residues 531 to 1144		FAD	Chemical				NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
60651	8	335630	7	NULL	NULL	0	NULL	iNOS	GP		bind			NOSred, residues 531 to 1144		NADPH	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
60652	9	335630	7	NULL	NULL	0	NULL	FMN	Chemical		is					flavin mononucleotide 	Chemical				NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
60653	10	335630	7	NULL	NULL	0	NULL	FAD	Chemical		is					flavin adenine dinucleotide	Chemical				NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
60654	11	335630	7	NULL	NULL	0	NULL	NOSox	GP		communicate with		electronically			NOSred	GP				NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
60655	12	335630	7	NULL	NULL	0	NULL	iNOS	GP		regulates			intervening calmodulin-binding region (residues 499 to 530)		statement 11	Process				NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
60656	13	335630	7	NULL	NULL	0	NULL	iron protoporphyrin IX	Chemical		is a type of					heme	Chemical				NULL		0	NULL	NULL	NULL	gw60_science_278_5337_425_s_22	9334294	NOS isozymes differ in size (130 to 160 kD), amino acid sequence (50 to 60% identity between any two isozymes), tissue distribution, transcriptional regulation, and activation by intracellular calcium ( 1), but they share an overall three-component construction ( 1,  2,  4,  5): (i) an NH2-terminal catalytic oxygenase domain (NOSox, residues 1 to 498 for iNOS) that binds heme (iron protoporphyrin IX), tetrahydrobiopterin (H4B), and the substrate L-Arg; (ii) a COOH-terminal reductase domain (NOSred, residues 531 to 1144 for iNOS) that binds flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), and NADPH; and (iii) an intervening calmodulin-binding region (residues 499 to 530 for iNOS) that regulates electronic communication between NOSox and NOSred ( 5,  9).	transcription
56253	1	335631	5	NULL	NULL	0	NULL	ATP			is transported to					mitochondrion					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
56254	2	335631	5	NULL	NULL	0	NULL	statement 1			via					translocase					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
56255	3	335631	5	NULL	NULL	0	NULL	translocase			is similar to					adenine nucleotide transporter					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
56256	4	335631	5	NULL	NULL	0	NULL	adenine nucleotide transporter			sensitive to					carboxyatractyloside					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
56257	5	335631	5	NULL	NULL	0	NULL	ATPase			is associated with					RIC					NULL	mitochondria	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
56258	6	335631	5	NULL	NULL	0	NULL	statement 5		activation of	catalyze					ATP		hydrolysis of			NULL	mitochondria	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
56259	7	335631	5	NULL	NULL	0	NULL	tRNA-receptor		binding of	leads to					statement 6					NULL	mitochondria 	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
56260	8	335631	5	NULL	NULL	0	NULL	protons			pumped from					membrane		inside			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
56261	9	335631	5	NULL	NULL	0	NULL	protons			pumped to					membrane		outside			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
56262	10	335631	5	NULL	NULL	0	NULL	statement 8			occurs simultaneously with					statement 9					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
56263	11	335631	5	NULL	NULL	0	NULL	statement 10			occurs through					oligomycin-sensitive channel					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
56264	12	335631	5	NULL	NULL	0	NULL	statement 10			generates					membrane potential					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
56265	13	335631	5	NULL	NULL	0	NULL	ATP		hydrolysis of	is accompanied by					statement 10					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
56266	14	335631	5	NULL	NULL	0	NULL	proton gradient		establishment of	opens					import channel					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
56267	15	335631	5	NULL	NULL	0	NULL	statement 14			occurs by		possibly			voltage gating					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
56268	16	335631	5	NULL	NULL	0	NULL	tRNA			transported through					import pore					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
60758	1	335631	7	NULL	NULL	0	NULL	ATP	Chemical		is transported into					mitochondrion	CellComponent				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
60759	2	335631	7	NULL	NULL	0	NULL	statement 1	Process		via					translocase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
60760	3	335631	7	NULL	NULL	0	NULL	translocase	GP		is similar to					carboxyatractyloside-sensitive adenine nucleotide transporter	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
60761	4	335631	7	NULL	NULL	0	NULL	RIC	GP		associate with					ATPase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
60762	5	335631	7	NULL	NULL	0	NULL	tRNA-receptor	GP	binding of	leads to					statement 4	Process	activation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
60763	6	335631	7	NULL	NULL	0	NULL	ATP	Chemical		hydrolyze within					mitochondrion	CellComponent				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
60764	7	335631	7	NULL	NULL	0	NULL	statement 4	Process		catalyze					statement 6	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
60766	8	335631	7	NULL	NULL	0	NULL	protons	Chemical		pumped from					inside membrane	CellComponent				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
60767	9	335631	7	NULL	NULL	0	NULL	protons	Chemical		pumped to					outside membrane	CellComponent				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
60769	10	335631	7	NULL	NULL	0	NULL	statement 8	Process		occur along with					statement 9	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
60770	11	335631	7	NULL	NULL	0	NULL	statement 10	Process		occur through					oligomycin-sensitive channel	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
60771	12	335631	7	NULL	NULL	0	NULL	statement 6	Process		is accompanied by					statement 10	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
60772	13	335631	7	NULL	NULL	0	NULL	statement 10	Process		result in					membrane potential	Process	generation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
60773	14	335631	7	NULL	NULL	0	NULL	Proton gradient	Process		leads to					import channel	CellComponent	opening of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
60774	15	335631	7	NULL	NULL	0	NULL	statement 14	Process		occur by		may			voltage gating	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
60775	16	335631	7	NULL	NULL	0	NULL	statement 15	Process		explain					deltapsi	Process	requirement of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
60776	17	335631	7	NULL	NULL	0	NULL	tRNA	NucleicAcid		is transported through					import pore	CellComponent				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
60777	18	335631	7	NULL	NULL	0	NULL	deltapsi	Process		is a type of					membrane potential	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_12_11259_s_142	14739289	Our current results are consistent with a multistep pathway of energy transduction within the complex leading, ultimately, to tRNA translocation; 1) substrate tRNA binds to its receptor; 2) ATP is transported into the mitochondrion via a translocase, which is similar or identical to the carboxyatractyloside-sensitive adenine nucleotide transporter; 3) tRNA-receptor binding leads to the activation of an RIC-associated ATPase which catalyzes ATP hydrolysis within the mitochondrion; 4) ATP hydrolysis is accompanied by pumping of protons through an oligomycin-sensitive channel from inside to outside the membrane, resulting in the generation of a membrane potential; 5) establishment of the proton gradient leads to opening of the import channel, possibly by voltage gating; this would explain the requirement for the membrane potential, deltapsi; 6) the tRNA is transported through the import pore.	transcription
58548	1	335632	5	NULL	NULL	0	NULL	target			undergoes					alteration					NULL	ribosomes	0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
58549	3	335632	5	NULL	NULL	0	NULL	statement 2			leads to					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
58550	2	335632	5	NULL	NULL	0	NULL	product of the erm gene			dimethylates					23S ribosomal RNA 				specific adenine residue \t	NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
58551	4	335632	5	NULL	NULL	0	NULL	statement 3			decreases					MLS antibiotics		binding of			NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
58552	5	335632	5	NULL	NULL	0	NULL	STG-B			is					streptogramin B					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
58553	6	335632	5	NULL	NULL	0	NULL	sbh gene			encodes					streptogramin B hydrolase					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
58554	7	335632	5	NULL	NULL	0	NULL	streptogramin B hydrolase			inactivates					STG-B					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
58555	8	335632	5	NULL	NULL	0	NULL	streptogramin B hydrolase			inactivates					lincosamide					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
58556	9	335632	5	NULL	NULL	0	NULL	linA''			encodes					3-lincomycin 4-clindamycin O-nucleotidyltransferase					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
58557	10	335632	5	NULL	NULL	0	NULL	3-lincomycin 4-clindamycin O-nucleotidyltransferase			inactivates					STG-B					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
58558	11	335632	5	NULL	NULL	0	NULL	3-lincomycin 4-clindamycin O-nucleotidyltransferase			inactivates					lincosamide					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
58559	12	335632	5	NULL	NULL	0	NULL	Mac antibiotics		active efflux of	determined by					msrA gene		Staphylococcus epidermidis			NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
58560	13	335632	5	NULL	NULL	0	NULL	STG-B antibiotics		active efflux of	determined by					msrB gene		Staphylococcus xylosus			NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
58561	15	335632	5	NULL	NULL	0	NULL	msrA gene		Staphylococcus epidermidis	acts as					statement 14					NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
58562	14	335632	5	NULL	NULL	0	NULL	efflux pump			is dependent on					ATP					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
58563	16	335632	5	NULL	NULL	0	NULL	msrB gene		Staphylococcus xylosus	acts as					statement 14					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
58564	17	335632	5	NULL	NULL	0	NULL	MLS antibiotics			is					macrolide, lincosamide, and streptogramin B antibiotics  					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
58565	18	335632	5	NULL	NULL	0	NULL	streptogramin B			is a type of					antibiotic					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
58566	19	335632	5	NULL	NULL	0	NULL	lincosamide			is a type of					antibiotic					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
58567	20	335632	5	NULL	NULL	0	NULL	macrolide			is a type of					antibiotic					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60778	1	335632	7	NULL	NULL	0	NULL	staphylococci 	Organism		resistant to					macrolide	Chemical				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60779	2	335632	7	NULL	NULL	0	NULL	staphylococci 	Organism		resistant to					lincosamide	Chemical				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60780	3	335632	7	NULL	NULL	0	NULL	staphylococci 	Organism		resistant to					streptogramin B	Chemical				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60781	4	335632	7	NULL	NULL	0	NULL	erm gene	GP	product of	dimethylates					adenine residues	NucleicAcid				NULL	23S ribosomal RNA	0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60782	5	335632	7	NULL	NULL	0	NULL	ribosome	CellComponent	alteration of target on	due to					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60783	6	335632	7	NULL	NULL	0	NULL	statement 5	Process		decrease					MLS antibiotics	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60784	7	335632	7	NULL	NULL	0	NULL	statement 5	Process		leads to					STG-B	Chemical	inactivation of			NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60785	8	335632	7	NULL	NULL	0	NULL	statement 5	Process		leads to					lincosamide	Chemical	inactivation of			NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60786	9	335632	7	NULL	NULL	0	NULL	sbh	GP		catalyze					statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60789	10	335632	7	NULL	NULL	0	NULL	linA	GP		catalyze					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60790	11	335632	7	NULL	NULL	0	NULL	sbh	GP		encode					streptogramin B hydrolase	GP				NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60791	12	335632	7	NULL	NULL	0	NULL	linA	GP		encode					3-lincomycin 4-clindamycin O-nucleotidyltransferase	GP				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60792	13	335632	7	NULL	NULL	0	NULL	STG-B	Chemical		is					streptogramin B	Chemical				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60799	14	335632	7	NULL	NULL	0	NULL	Mac	Chemical	active efflux of	determined by					msrA gene					NULL	Staphylococcus epidermidis	NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60808	15	335632	7	NULL	NULL	0	NULL	STG-B antibiotics	Chemical	active efflux of	determined by					msrB genes	GP				NULL	Staphylococcus xylosus	0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60811	16	335632	7	NULL	NULL	0	NULL	Mac	Chemical	active efflux of	act as					ATP-dependent efflux pumps	Process				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60812	17	335632	7	NULL	NULL	0	NULL	STG-B antibiotics	Chemical	active efflux of	act as					ATP-dependent efflux pumps	Process				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60813	18	335632	7	NULL	NULL	0	NULL	statement 1	Process		reflect					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60814	19	335632	7	NULL	NULL	0	NULL	statement 2	Process		reflect					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60815	20	335632	7	NULL	NULL	0	NULL	statement 3	Process		reflect					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60816	21	335632	7	NULL	NULL	0	NULL	statement 1	Process		reflect					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60817	22	335632	7	NULL	NULL	0	NULL	statement 2	Process		reflect					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60818	23	335632	7	NULL	NULL	0	NULL	statement 3	Process		reflect					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60819	24	335632	7	NULL	NULL	0	NULL	statement 1	Process		reflect					statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60820	25	335632	7	NULL	NULL	0	NULL	statement 2	Process		reflect					statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60821	26	335632	7	NULL	NULL	0	NULL	statement 3	Process		reflect					statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60822	27	335632	7	NULL	NULL	0	NULL	statement 1	Process		reflect					statement 8	Process				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60823	28	335632	7	NULL	NULL	0	NULL	statement 2	Process		reflect					statement 8	Process				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60824	29	335632	7	NULL	NULL	0	NULL	statement 3	Process		reflect					statement 8	Process				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60825	30	335632	7	NULL	NULL	0	NULL	statement 1	Process		reflect					statement 16	Process				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60826	31	335632	7	NULL	NULL	0	NULL	statement 2	Process		reflect					statement 16	Process				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60827	32	335632	7	NULL	NULL	0	NULL	statement 3	Process		reflect					statement 16	Process				NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60828	33	335632	7	NULL	NULL	0	NULL	statement 1	Process		reflect					statement 17	Process				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60829	34	335632	7	NULL	NULL	0	NULL	statement 2	Process		reflect					statement 17	Process				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
60830	35	335632	7	NULL	NULL	0	NULL	statement 3	Process		reflect					statement 17	Process				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_181_1_91_s_6	10564793	Resistance to macrolide, lincosamide, and streptogramin B (MLS) antibiotics in staphylococci is known to have the following mechanisms: (1) alteration of the target on ribosome due to dimethylation of a specific adenine residue in the 23S ribosomal RNA by the product of the  erm gene, and consequently a decrease in binding of MLS antibiotics [  4,   5 and   6]; (2) inactivation of streptogramin B (STG-B) and lincosamide by the products of the  sbh (encoding streptogramin B hydrolase) [  7] and  linA'' (encoding 3-lincomycin 4-clindamycin  O-nucleotidyltransferase) [  8 genes, respectively; and (3) active efflux of Mac and STG-B antibiotics determined by the  msrA and  msrB genes in  Staphylococcus epidermidis and  Staphylococcus xylosus, respectively [  9 and   10], both of which appear to act as ATP-dependent efflux pumps.	transcription
56269	1	335634	5	NULL	NULL	0	NULL	choline			is oxidized to					glycine-betaine					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_36	12676692	Oxidation of choline to glycine-betaine catalyzed by choline dehydrogenase.	transcription
56270	2	335634	5	NULL	NULL	0	NULL	choline dehydrogenase			catalyze					statement 1					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_36	12676692	Oxidation of choline to glycine-betaine catalyzed by choline dehydrogenase.	transcription
60831	1	335634	7	NULL	NULL	0	NULL	choline	Chemical		oxidizes to					glycine-betaine	AminoAcid				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_36	12676692	Oxidation of choline to glycine-betaine catalyzed by choline dehydrogenase.	transcription
60832	2	335634	7	NULL	NULL	0	NULL	choline dehydrogenase	GP		catalyze					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_36	12676692	Oxidation of choline to glycine-betaine catalyzed by choline dehydrogenase.	transcription
56271	1	335635	5	NULL	NULL	0	NULL	choline			is converted to					glycine betaine					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_7_2273_s_62	10094709	CudA and CudB catalyze the conversion of choline to glycine betaine.	transcription
56272	2	335635	5	NULL	NULL	0	NULL	CudB			catalyze					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_7_2273_s_62	10094709	CudA and CudB catalyze the conversion of choline to glycine betaine.	transcription
56273	3	335635	5	NULL	NULL	0	NULL	CudA			catalyze					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_7_2273_s_62	10094709	CudA and CudB catalyze the conversion of choline to glycine betaine.	transcription
60833	1	335635	7	NULL	NULL	0	NULL	choline	Chemical		converted to					glycine betaine	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbacteriol_181_7_2273_s_62	10094709	CudA and CudB catalyze the conversion of choline to glycine betaine.	transcription
60834	2	335635	7	NULL	NULL	0	NULL	CudA 	GP		catalyze					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_7_2273_s_62	10094709	CudA and CudB catalyze the conversion of choline to glycine betaine.	transcription
60835	3	335635	7	NULL	NULL	0	NULL	CudB	GP		catalyze					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbacteriol_181_7_2273_s_62	10094709	CudA and CudB catalyze the conversion of choline to glycine betaine.	transcription
56274	1	335636	5	NULL	NULL	0	NULL	bet genes			is induced by					choline					NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_50_0_101_s_158	8905077	The  bet genes are also induced by choline and repressed by glycine betaine.	transcription
56275	2	335636	5	NULL	NULL	0	NULL	bet genes			repressed by					glycine betaine					NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_50_0_101_s_158	8905077	The  bet genes are also induced by choline and repressed by glycine betaine.	transcription
60836	1	335636	7	NULL	NULL	0	NULL	 choline	Chemical		induce					bet genes	GP				NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_50_0_101_s_158	8905077	The  bet genes are also induced by choline and repressed by glycine betaine.	transcription
60837	2	335636	7	NULL	NULL	0	NULL	glycine betaine	AminoAcid		repress					bet genes	GP				NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_50_0_101_s_158	8905077	The  bet genes are also induced by choline and repressed by glycine betaine.	transcription
56276	1	335637	5	NULL	NULL	0	NULL	choline			is oxidized to					glycine betaine					NULL	cytoplasm	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1420_1_30_s_18	10446288	Enzymes BetB and BetA catalyze the cytoplasmic oxidation of choline to glycine betaine.	transcription
56277	2	335637	5	NULL	NULL	0	NULL	BetB enzyme			catalyze					statement 1					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1420_1_30_s_18	10446288	Enzymes BetB and BetA catalyze the cytoplasmic oxidation of choline to glycine betaine.	transcription
56278	3	335637	5	NULL	NULL	0	NULL	BetA enzyme			catalyze					statement 1					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1420_1_30_s_18	10446288	Enzymes BetB and BetA catalyze the cytoplasmic oxidation of choline to glycine betaine.	transcription
60838	1	335637	7	NULL	NULL	0	NULL	Choline	Chemical		oxidizes to					glycine betaine	AminoAcid				NULL	cytoplasm	0	NULL	NULL	NULL	gw60_biochimbiophysacta_1420_1_30_s_18	10446288	Enzymes BetB and BetA catalyze the cytoplasmic oxidation of choline to glycine betaine.	transcription
60839	2	335637	7	NULL	NULL	0	NULL	BetB	GP		catalyze					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1420_1_30_s_18	10446288	Enzymes BetB and BetA catalyze the cytoplasmic oxidation of choline to glycine betaine.	transcription
60840	3	335637	7	NULL	NULL	0	NULL	BetA	GP		catalyze					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1420_1_30_s_18	10446288	Enzymes BetB and BetA catalyze the cytoplasmic oxidation of choline to glycine betaine.	transcription
56279	1	335638	5	NULL	NULL	0	NULL	choline			is oxidized to					glycine-betaine					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_2_296_s_131	14702297	Choline is an osmoprotectant for  E. coli K-12 because BetT mediates choline uptake while BetB and BetA mediate choline oxidation to glycine-betaine ( ).	transcription
56280	2	335638	5	NULL	NULL	0	NULL	BetB			mediates					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_2_296_s_131	14702297	Choline is an osmoprotectant for  E. coli K-12 because BetT mediates choline uptake while BetB and BetA mediate choline oxidation to glycine-betaine ( ).	transcription
56281	3	335638	5	NULL	NULL	0	NULL	BetA			mediates					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_2_296_s_131	14702297	Choline is an osmoprotectant for  E. coli K-12 because BetT mediates choline uptake while BetB and BetA mediate choline oxidation to glycine-betaine ( ).	transcription
56282	4	335638	5	NULL	NULL	0	NULL	BetT			mediates					choline		uptake of			NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_2_296_s_131	14702297	Choline is an osmoprotectant for  E. coli K-12 because BetT mediates choline uptake while BetB and BetA mediate choline oxidation to glycine-betaine ( ).	transcription
56283	5	335638	5	NULL	NULL	0	NULL	choline			acts as					osmoprotectant		E. coli K-12			NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_2_296_s_131	14702297	Choline is an osmoprotectant for  E. coli K-12 because BetT mediates choline uptake while BetB and BetA mediate choline oxidation to glycine-betaine ( ).	transcription
60841	1	335638	7	NULL	NULL	0	NULL	choline	Chemical		is a type of					osmoprotectant	Chemical				NULL	E. coli K-12	0	NULL	NULL	NULL	gw70_jbacteriol_186_2_296_s_131	14702297	Choline is an osmoprotectant for  E. coli K-12 because BetT mediates choline uptake while BetB and BetA mediate choline oxidation to glycine-betaine ( ).	transcription
60842	2	335638	7	NULL	NULL	0	NULL	BetT	GP		mediates					choline	Chemical	uptake of			NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_2_296_s_131	14702297	Choline is an osmoprotectant for  E. coli K-12 because BetT mediates choline uptake while BetB and BetA mediate choline oxidation to glycine-betaine ( ).	transcription
60843	3	335638	7	NULL	NULL	0	NULL	statement 1	Process		because of					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_2_296_s_131	14702297	Choline is an osmoprotectant for  E. coli K-12 because BetT mediates choline uptake while BetB and BetA mediate choline oxidation to glycine-betaine ( ).	transcription
60844	4	335638	7	NULL	NULL	0	NULL	choline	Chemical		oxidizes to					glycine-betaine	Aminoacid				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_2_296_s_131	14702297	Choline is an osmoprotectant for  E. coli K-12 because BetT mediates choline uptake while BetB and BetA mediate choline oxidation to glycine-betaine ( ).	transcription
60845	5	335638	7	NULL	NULL	0	NULL	BetB	GP		mediate					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_2_296_s_131	14702297	Choline is an osmoprotectant for  E. coli K-12 because BetT mediates choline uptake while BetB and BetA mediate choline oxidation to glycine-betaine ( ).	transcription
60846	6	335638	7	NULL	NULL	0	NULL	BetA	GP		mediate					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_2_296_s_131	14702297	Choline is an osmoprotectant for  E. coli K-12 because BetT mediates choline uptake while BetB and BetA mediate choline oxidation to glycine-betaine ( ).	transcription
56284	1	335639	5	NULL	NULL	0	NULL	choline sulfate			hydrolyzed to					choline					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiolrev_24_2_135_s_349	10717312	The BetC protein catalyzes the hydrolysis of choline sulfate to choline, and is part of a pathway that synthesizes the osmoprotectant glycine betaine.	transcription
56285	2	335639	5	NULL	NULL	0	NULL	BetC protein			catalyze					statement 1					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiolrev_24_2_135_s_349	10717312	The BetC protein catalyzes the hydrolysis of choline sulfate to choline, and is part of a pathway that synthesizes the osmoprotectant glycine betaine.	transcription
56286	3	335639	5	NULL	NULL	0	NULL	glycine betaine			is a type of					osmoprotectant					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiolrev_24_2_135_s_349	10717312	The BetC protein catalyzes the hydrolysis of choline sulfate to choline, and is part of a pathway that synthesizes the osmoprotectant glycine betaine.	transcription
56287	4	335639	5	NULL	NULL	0	NULL	BetC protein			plays a role in					glycine betaine		synthesis of			NULL		0	NULL	NULL	NULL	gw60_femsmicrobiolrev_24_2_135_s_349	10717312	The BetC protein catalyzes the hydrolysis of choline sulfate to choline, and is part of a pathway that synthesizes the osmoprotectant glycine betaine.	transcription
60847	1	335639	7	NULL	NULL	0	NULL	choline sulfate	Chemical		hydrolyze to					Choline	Chemical				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiolrev_24_2_135_s_349	10717312	The BetC protein catalyzes the hydrolysis of choline sulfate to choline, and is part of a pathway that synthesizes the osmoprotectant glycine betaine.	transcription
60848	2	335639	7	NULL	NULL	0	NULL	BetC protein 	GP		catalyze					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiolrev_24_2_135_s_349	10717312	The BetC protein catalyzes the hydrolysis of choline sulfate to choline, and is part of a pathway that synthesizes the osmoprotectant glycine betaine.	transcription
60849	3	335639	7	NULL	NULL	0	NULL	BetC protein 	GP		is part of					glycine betaine	AminoAcid	pathway that synthesizes			NULL		0	NULL	NULL	NULL	gw60_femsmicrobiolrev_24_2_135_s_349	10717312	The BetC protein catalyzes the hydrolysis of choline sulfate to choline, and is part of a pathway that synthesizes the osmoprotectant glycine betaine.	transcription
60850	4	335639	7	NULL	NULL	0	NULL	glycine betaine	AminoAcid		is a type of					osmoprotectant	Chemical				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiolrev_24_2_135_s_349	10717312	The BetC protein catalyzes the hydrolysis of choline sulfate to choline, and is part of a pathway that synthesizes the osmoprotectant glycine betaine.	transcription
56288	1	335640	5	NULL	NULL	0	NULL	choline			is oxidized to					glycine betaine					NULL		0	NULL	NULL	NULL	abs-batch0550-0559_j-am-chem-soc_127_50_16351127_s_2	16351127	Choline oxidase catalyzes the flavin-linked oxidation of choline to glycine  betaine, with betaine aldehyde as intermediate and oxygen as electron  acceptor.	transcription
56289	2	335640	5	NULL	NULL	0	NULL	statement 1			linked to					flavin					NULL		0	NULL	NULL	NULL	abs-batch0550-0559_j-am-chem-soc_127_50_16351127_s_2	16351127	Choline oxidase catalyzes the flavin-linked oxidation of choline to glycine  betaine, with betaine aldehyde as intermediate and oxygen as electron  acceptor.	transcription
56290	3	335640	5	NULL	NULL	0	NULL	choline oxidase			catalyze					statement 1					NULL		0	NULL	NULL	NULL	abs-batch0550-0559_j-am-chem-soc_127_50_16351127_s_2	16351127	Choline oxidase catalyzes the flavin-linked oxidation of choline to glycine  betaine, with betaine aldehyde as intermediate and oxygen as electron  acceptor.	transcription
56291	4	335640	5	NULL	NULL	0	NULL	betaine aldehyde			is produced as					intermediate					NULL		0	NULL	NULL	NULL	abs-batch0550-0559_j-am-chem-soc_127_50_16351127_s_2	16351127	Choline oxidase catalyzes the flavin-linked oxidation of choline to glycine  betaine, with betaine aldehyde as intermediate and oxygen as electron  acceptor.	transcription
56292	5	335640	5	NULL	NULL	0	NULL	statement 4			occurs simultaneously with					statement 1					NULL		0	NULL	NULL	NULL	abs-batch0550-0559_j-am-chem-soc_127_50_16351127_s_2	16351127	Choline oxidase catalyzes the flavin-linked oxidation of choline to glycine  betaine, with betaine aldehyde as intermediate and oxygen as electron  acceptor.	transcription
56293	6	335640	5	NULL	NULL	0	NULL	oxygen			acts as					electron acceptor					NULL		0	NULL	NULL	NULL	abs-batch0550-0559_j-am-chem-soc_127_50_16351127_s_2	16351127	Choline oxidase catalyzes the flavin-linked oxidation of choline to glycine  betaine, with betaine aldehyde as intermediate and oxygen as electron  acceptor.	transcription
60851	1	335640	7	NULL	NULL	0	NULL	Choline	Chemical		oxidizes to					glycine betaine	AminoAcid				NULL		0	NULL	NULL	NULL	abs-batch0550-0559_j-am-chem-soc_127_50_16351127_s_2	16351127	Choline oxidase catalyzes the flavin-linked oxidation of choline to glycine  betaine, with betaine aldehyde as intermediate and oxygen as electron  acceptor.	transcription
60852	2	335640	7	NULL	NULL	0	NULL	Choline oxidase	GP		catalyze					statement 1	Process	flavin-linked oxidation of			NULL		0	NULL	NULL	NULL	abs-batch0550-0559_j-am-chem-soc_127_50_16351127_s_2	16351127	Choline oxidase catalyzes the flavin-linked oxidation of choline to glycine  betaine, with betaine aldehyde as intermediate and oxygen as electron  acceptor.	transcription
60853	3	335640	7	NULL	NULL	0	NULL	betaine aldehyde	Chemical		acts as a					statement 1	Chemical	intermediate of			NULL		NULL	NULL	NULL	NULL	abs-batch0550-0559_j-am-chem-soc_127_50_16351127_s_2	16351127	Choline oxidase catalyzes the flavin-linked oxidation of choline to glycine  betaine, with betaine aldehyde as intermediate and oxygen as electron  acceptor.	transcription
60854	4	335640	7	NULL	NULL	0	NULL	oxygen	Chemical		acts as a					statement 1	Process	electron acceptor of			NULL		0	NULL	NULL	NULL	abs-batch0550-0559_j-am-chem-soc_127_50_16351127_s_2	16351127	Choline oxidase catalyzes the flavin-linked oxidation of choline to glycine  betaine, with betaine aldehyde as intermediate and oxygen as electron  acceptor.	transcription
56294	1	335641	5	NULL	NULL	0	NULL	choline			is oxidized to					glycine betaine					NULL		0	NULL	NULL	NULL	abs-batch0600-0619_biochemistry_45_6_16460045_s_2	16460045	Choline oxidase catalyzes the four-electron oxidation of choline to glycine  betaine via two sequential FAD-dependent reactions in which betaine aldehyde  is formed as an intermediate.	transcription
56295	2	335641	5	NULL	NULL	0	NULL	statement 1			via					FAD-dependent reactions		sequential			NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_biochemistry_45_6_16460045_s_2	16460045	Choline oxidase catalyzes the four-electron oxidation of choline to glycine  betaine via two sequential FAD-dependent reactions in which betaine aldehyde  is formed as an intermediate.	transcription
56296	3	335641	5	NULL	NULL	0	NULL	choline oxidase			catalyze					statement 1					NULL		0	NULL	NULL	NULL	abs-batch0600-0619_biochemistry_45_6_16460045_s_2	16460045	Choline oxidase catalyzes the four-electron oxidation of choline to glycine  betaine via two sequential FAD-dependent reactions in which betaine aldehyde  is formed as an intermediate.	transcription
56297	4	335641	5	NULL	NULL	0	NULL	betaine aldehyde			formed as					intermediate					NULL		0	NULL	NULL	NULL	abs-batch0600-0619_biochemistry_45_6_16460045_s_2	16460045	Choline oxidase catalyzes the four-electron oxidation of choline to glycine  betaine via two sequential FAD-dependent reactions in which betaine aldehyde  is formed as an intermediate.	transcription
56298	5	335641	5	NULL	NULL	0	NULL	statement 4			occurs simultaneously with					statement 1					NULL		0	NULL	NULL	NULL	abs-batch0600-0619_biochemistry_45_6_16460045_s_2	16460045	Choline oxidase catalyzes the four-electron oxidation of choline to glycine  betaine via two sequential FAD-dependent reactions in which betaine aldehyde  is formed as an intermediate.	transcription
60855	1	335641	7	NULL	NULL	0	NULL	choline	Chemical		oxidizes to					glycine betaine	AminoAcid				NULL		0	NULL	NULL	NULL	abs-batch0600-0619_biochemistry_45_6_16460045_s_2	16460045	Choline oxidase catalyzes the four-electron oxidation of choline to glycine  betaine via two sequential FAD-dependent reactions in which betaine aldehyde  is formed as an intermediate.	transcription
60856	2	335641	7	NULL	NULL	0	NULL	Choline oxidase	GP		catalyze					statement 1	Process	four-electron oxidation of			NULL		0	NULL	NULL	NULL	abs-batch0600-0619_biochemistry_45_6_16460045_s_2	16460045	Choline oxidase catalyzes the four-electron oxidation of choline to glycine  betaine via two sequential FAD-dependent reactions in which betaine aldehyde  is formed as an intermediate.	transcription
60857	3	335641	7	NULL	NULL	0	NULL	statement 2	Process		via					sequential FAD-dependent reactions	Process				NULL		0	NULL	NULL	NULL	abs-batch0600-0619_biochemistry_45_6_16460045_s_2	16460045	Choline oxidase catalyzes the four-electron oxidation of choline to glycine  betaine via two sequential FAD-dependent reactions in which betaine aldehyde  is formed as an intermediate.	transcription
60858	4	335641	7	NULL	NULL	0	NULL	betaine aldehyde	Chemical		is formed as a					statement 1	Process	intermediate of			NULL		0	NULL	NULL	NULL	abs-batch0600-0619_biochemistry_45_6_16460045_s_2	16460045	Choline oxidase catalyzes the four-electron oxidation of choline to glycine  betaine via two sequential FAD-dependent reactions in which betaine aldehyde  is formed as an intermediate.	transcription
56299	1	335642	5	NULL	NULL	0	NULL	choline			is converted to					glycine betaine					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_6_1683_s_137	14996799	To test whether the thermoprotective effect of choline was dependent on its GbsA- and GbsB-mediated enzymatic conversion to glycine betaine ( ), we grew the delta( gbsAB:: neo) 2 strain JBB5 in the presence of either glycine betaine or choline.	transcription
56300	2	335642	5	NULL	NULL	0	NULL	GbsA enzyme			mediates					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_6_1683_s_137	14996799	To test whether the thermoprotective effect of choline was dependent on its GbsA- and GbsB-mediated enzymatic conversion to glycine betaine ( ), we grew the delta( gbsAB:: neo) 2 strain JBB5 in the presence of either glycine betaine or choline.	transcription
56301	3	335642	5	NULL	NULL	0	NULL	GbsB enzyme			mediates					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_6_1683_s_137	14996799	To test whether the thermoprotective effect of choline was dependent on its GbsA- and GbsB-mediated enzymatic conversion to glycine betaine ( ), we grew the delta( gbsAB:: neo) 2 strain JBB5 in the presence of either glycine betaine or choline.	transcription
56302	4	335642	5	NULL	NULL	0	NULL	choline		thermoprotective effect of	is dependent on		possibly			statement 2					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_6_1683_s_137	14996799	To test whether the thermoprotective effect of choline was dependent on its GbsA- and GbsB-mediated enzymatic conversion to glycine betaine ( ), we grew the delta( gbsAB:: neo) 2 strain JBB5 in the presence of either glycine betaine or choline.	transcription
56303	5	335642	5	NULL	NULL	0	NULL	choline		thermoprotective effect of	is dependent on		possibly			statement 3					NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_6_1683_s_137	14996799	To test whether the thermoprotective effect of choline was dependent on its GbsA- and GbsB-mediated enzymatic conversion to glycine betaine ( ), we grew the delta( gbsAB:: neo) 2 strain JBB5 in the presence of either glycine betaine or choline.	transcription
60859	1	335642	7	NULL	NULL	0	NULL	GbsA	GP		mediate					glycine betaine	AminoAcid	enzymatic conversion to			NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_6_1683_s_137	14996799	To test whether the thermoprotective effect of choline was dependent on its GbsA- and GbsB-mediated enzymatic conversion to glycine betaine ( ), we grew the delta( gbsAB:: neo) 2 strain JBB5 in the presence of either glycine betaine or choline.	transcription
60860	2	335642	7	NULL	NULL	0	NULL	GbsB	GP		mediate					glycine betaine	AminoAcid	enzymatic conversion to			NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_6_1683_s_137	14996799	To test whether the thermoprotective effect of choline was dependent on its GbsA- and GbsB-mediated enzymatic conversion to glycine betaine ( ), we grew the delta( gbsAB:: neo) 2 strain JBB5 in the presence of either glycine betaine or choline.	transcription
56314	1	335643	5	NULL	NULL	0	NULL	BetB			is					choline dehydrogenase					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_28_20011_s_74	10391951	The proposed pathway of choline degradation ( 17) is initiated by two subsequent oxidation steps catalyzed by choline dehydrogenase (BetB) and glycine betaine aldehyde dehydrogenase (BetA) leading to the formation of glycine betaine, which can be metabolized further ( 16).	transcription
56315	2	335643	5	NULL	NULL	0	NULL	BetA			is					glycine betaine aldehyde dehydrogenase					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_28_20011_s_74	10391951	The proposed pathway of choline degradation ( 17) is initiated by two subsequent oxidation steps catalyzed by choline dehydrogenase (BetB) and glycine betaine aldehyde dehydrogenase (BetA) leading to the formation of glycine betaine, which can be metabolized further ( 16).	transcription
56316	3	335643	5	NULL	NULL	0	NULL	BetB			catalyze					glycine betaine		formation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_28_20011_s_74	10391951	The proposed pathway of choline degradation ( 17) is initiated by two subsequent oxidation steps catalyzed by choline dehydrogenase (BetB) and glycine betaine aldehyde dehydrogenase (BetA) leading to the formation of glycine betaine, which can be metabolized further ( 16).	transcription
56317	4	335643	5	NULL	NULL	0	NULL	BetA			catalyze					glycine betaine		formation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_28_20011_s_74	10391951	The proposed pathway of choline degradation ( 17) is initiated by two subsequent oxidation steps catalyzed by choline dehydrogenase (BetB) and glycine betaine aldehyde dehydrogenase (BetA) leading to the formation of glycine betaine, which can be metabolized further ( 16).	transcription
56318	5	335643	5	NULL	NULL	0	NULL	statement 3			subsequent to					statement 4					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_28_20011_s_74	10391951	The proposed pathway of choline degradation ( 17) is initiated by two subsequent oxidation steps catalyzed by choline dehydrogenase (BetB) and glycine betaine aldehyde dehydrogenase (BetA) leading to the formation of glycine betaine, which can be metabolized further ( 16).	transcription
56319	6	335643	5	NULL	NULL	0	NULL	statement 5			initiates					choline degradation pathway					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_28_20011_s_74	10391951	The proposed pathway of choline degradation ( 17) is initiated by two subsequent oxidation steps catalyzed by choline dehydrogenase (BetB) and glycine betaine aldehyde dehydrogenase (BetA) leading to the formation of glycine betaine, which can be metabolized further ( 16).	transcription
56320	7	335643	5	NULL	NULL	0	NULL	glycine betaine			undergoes					metabolism					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_28_20011_s_74	10391951	The proposed pathway of choline degradation ( 17) is initiated by two subsequent oxidation steps catalyzed by choline dehydrogenase (BetB) and glycine betaine aldehyde dehydrogenase (BetA) leading to the formation of glycine betaine, which can be metabolized further ( 16).	transcription
60861	1	335643	7	NULL	NULL	0	NULL	choline 	Chemical		degraded to					glycine betaine	AminoAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_28_20011_s_74	10391951	The proposed pathway of choline degradation ( 17) is initiated by two subsequent oxidation steps catalyzed by choline dehydrogenase (BetB) and glycine betaine aldehyde dehydrogenase (BetA) leading to the formation of glycine betaine, which can be metabolized further ( 16).	transcription
60862	2	335643	7	NULL	NULL	0	NULL	choline dehydrogenase	GP		catalyze					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_28_20011_s_74	10391951	The proposed pathway of choline degradation ( 17) is initiated by two subsequent oxidation steps catalyzed by choline dehydrogenase (BetB) and glycine betaine aldehyde dehydrogenase (BetA) leading to the formation of glycine betaine, which can be metabolized further ( 16).	transcription
60863	3	335643	7	NULL	NULL	0	NULL	glycine betaine aldehyde dehydrogenase 	GP		catalyze					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_28_20011_s_74	10391951	The proposed pathway of choline degradation ( 17) is initiated by two subsequent oxidation steps catalyzed by choline dehydrogenase (BetB) and glycine betaine aldehyde dehydrogenase (BetA) leading to the formation of glycine betaine, which can be metabolized further ( 16).	transcription
60864	4	335643	7	NULL	NULL	0	NULL	BetB	GP		is					choline dehydrogenase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_28_20011_s_74	10391951	The proposed pathway of choline degradation ( 17) is initiated by two subsequent oxidation steps catalyzed by choline dehydrogenase (BetB) and glycine betaine aldehyde dehydrogenase (BetA) leading to the formation of glycine betaine, which can be metabolized further ( 16).	transcription
60865	5	335643	7	NULL	NULL	0	NULL	BetA	GP		is					glycine betaine aldehyde dehydrogenase 	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_28_20011_s_74	10391951	The proposed pathway of choline degradation ( 17) is initiated by two subsequent oxidation steps catalyzed by choline dehydrogenase (BetB) and glycine betaine aldehyde dehydrogenase (BetA) leading to the formation of glycine betaine, which can be metabolized further ( 16).	transcription
60866	6	335643	7	NULL	NULL	0	NULL	statement 2	Process		is a type of					oxidation step	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_28_20011_s_74	10391951	The proposed pathway of choline degradation ( 17) is initiated by two subsequent oxidation steps catalyzed by choline dehydrogenase (BetB) and glycine betaine aldehyde dehydrogenase (BetA) leading to the formation of glycine betaine, which can be metabolized further ( 16).	transcription
60867	7	335643	7	NULL	NULL	0	NULL	statement 3	Process		is a type of					oxidation step	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_28_20011_s_74	10391951	The proposed pathway of choline degradation ( 17) is initiated by two subsequent oxidation steps catalyzed by choline dehydrogenase (BetB) and glycine betaine aldehyde dehydrogenase (BetA) leading to the formation of glycine betaine, which can be metabolized further ( 16).	transcription
60868	1	335645	7	NULL	NULL	0	NULL	fixA-lacZ transcriptional fusion	GP	expression of	induced by					l-carnitine	Chemical				NULL		0	NULL	NULL	NULL	gw70_annurevnutr_18_0_39_s_114	9706218	Expression of a  fixA-lacZ transcriptional fusion was induced by  l-carnitine and crotonobetaine, but not by  d-carnitine,  -butyrobetaine, glycine betaine, or choline.	transcription
60869	2	335645	7	NULL	NULL	0	NULL	fixA-lacZ transcriptional fusion	GP	expression of	induced by					crotonobetaine	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_annurevnutr_18_0_39_s_114	9706218	Expression of a  fixA-lacZ transcriptional fusion was induced by  l-carnitine and crotonobetaine, but not by  d-carnitine,  -butyrobetaine, glycine betaine, or choline.	transcription
60870	3	335645	7	NULL	NULL	0	NULL	d-carnitine	Chemical		does not induce					fixA-lacZ transcriptional fusion	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_annurevnutr_18_0_39_s_114	9706218	Expression of a  fixA-lacZ transcriptional fusion was induced by  l-carnitine and crotonobetaine, but not by  d-carnitine,  -butyrobetaine, glycine betaine, or choline.	transcription
60871	4	335645	7	NULL	NULL	0	NULL	butyrobetaine	Chemical		does not induce					fixA-lacZ transcriptional fusion	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_annurevnutr_18_0_39_s_114	9706218	Expression of a  fixA-lacZ transcriptional fusion was induced by  l-carnitine and crotonobetaine, but not by  d-carnitine,  -butyrobetaine, glycine betaine, or choline.	transcription
60872	5	335645	7	NULL	NULL	0	NULL	glycine betaine	AminoAcid		does not induce					fixA-lacZ transcriptional fusion	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_annurevnutr_18_0_39_s_114	9706218	Expression of a  fixA-lacZ transcriptional fusion was induced by  l-carnitine and crotonobetaine, but not by  d-carnitine,  -butyrobetaine, glycine betaine, or choline.	transcription
60873	6	335645	7	NULL	NULL	0	NULL	choline	Chemical		does not induce					fixA-lacZ transcriptional fusion	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_annurevnutr_18_0_39_s_114	9706218	Expression of a  fixA-lacZ transcriptional fusion was induced by  l-carnitine and crotonobetaine, but not by  d-carnitine,  -butyrobetaine, glycine betaine, or choline.	transcription
56321	1	335646	5	NULL	NULL	0	NULL	choline			is oxidized to					glycine betaine					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_3	12676692	99.1) catalyzes the four-electron oxidation of choline to glycine-betaine via a betaine-aldehyde intermediate.	transcription
56322	2	335646	5	NULL	NULL	0	NULL	statement 1			via					betaine-aldehyde intermediate					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_3	12676692	99.1) catalyzes the four-electron oxidation of choline to glycine-betaine via a betaine-aldehyde intermediate.	transcription
60874	1	335646	7	NULL	NULL	0	NULL	choline	Chemical		oxidizes to					glycine-betaine	AminoAcid				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_3	12676692	99.1) catalyzes the four-electron oxidation of choline to glycine-betaine via a betaine-aldehyde intermediate.	transcription
60875	2	335646	7	NULL	NULL	0	NULL	statement 1	Process		via					betaine-aldehyde intermediate	Chemical				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_3	12676692	99.1) catalyzes the four-electron oxidation of choline to glycine-betaine via a betaine-aldehyde intermediate.	transcription
56323	1	335647	5	NULL	NULL	0	NULL	ABC transporters			mediates					choline		uptake of			NULL	Bacillus subtilis	NULL	NULL	NULL	NULL	gw60_genomeres_11_9_1484_s_448	11544192	Two evolutionarily closely related ABC transporters mediate the uptake of choline for synthesis of the osmoprotectant glycine betaine in  Bacillus subtilis.	transcription
56324	2	335647	5	NULL	NULL	0	NULL	statement 1			is required for					glycine betaine		synthesis of			NULL	Bacillus subtilis	0	NULL	NULL	NULL	gw60_genomeres_11_9_1484_s_448	11544192	Two evolutionarily closely related ABC transporters mediate the uptake of choline for synthesis of the osmoprotectant glycine betaine in  Bacillus subtilis.	transcription
56325	3	335647	5	NULL	NULL	0	NULL	glycine betaine			is a type of					osmoprotectant					NULL		0	NULL	NULL	NULL	gw60_genomeres_11_9_1484_s_448	11544192	Two evolutionarily closely related ABC transporters mediate the uptake of choline for synthesis of the osmoprotectant glycine betaine in  Bacillus subtilis.	transcription
60876	1	335647	7	NULL	NULL	0	NULL	ABC transporters	GP		mediate					choline	Chemical	uptake of			NULL	Bacillus subtilis	NULL	NULL	NULL	NULL	gw60_genomeres_11_9_1484_s_448	11544192	Two evolutionarily closely related ABC transporters mediate the uptake of choline for synthesis of the osmoprotectant glycine betaine in  Bacillus subtilis.	transcription
60877	2	335647	7	NULL	NULL	0	NULL	statement 1	Process		for synthesis of					glycine betaine	AminoAcid				NULL	Bacillus subtilis	0	NULL	NULL	NULL	gw60_genomeres_11_9_1484_s_448	11544192	Two evolutionarily closely related ABC transporters mediate the uptake of choline for synthesis of the osmoprotectant glycine betaine in  Bacillus subtilis.	transcription
60878	3	335647	7	NULL	NULL	0	NULL	glycine betaine	AminoAcid		is a type of					osmoprotectant	AminoAcid				NULL		0	NULL	NULL	NULL	gw60_genomeres_11_9_1484_s_448	11544192	Two evolutionarily closely related ABC transporters mediate the uptake of choline for synthesis of the osmoprotectant glycine betaine in  Bacillus subtilis.	transcription
56326	1	335650	5	NULL	NULL	0	NULL	glycine			induces					steady-state currents					NULL	wild type transporters	0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13856_s_174	10788509	Replacement of sodium by choline abolished glycine induced steady-state currents in wild type and mutant transporters.	transcription
56327	2	335650	5	NULL	NULL	0	NULL	glycine			induces					steady-state currents					NULL	mutant transporters	0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13856_s_174	10788509	Replacement of sodium by choline abolished glycine induced steady-state currents in wild type and mutant transporters.	transcription
56328	3	335650	5	NULL	NULL	0	NULL	sodium			is replaced with					choline					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13856_s_174	10788509	Replacement of sodium by choline abolished glycine induced steady-state currents in wild type and mutant transporters.	transcription
56329	4	335650	5	NULL	NULL	0	NULL	statement 3			abolishes					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13856_s_174	10788509	Replacement of sodium by choline abolished glycine induced steady-state currents in wild type and mutant transporters.	transcription
56330	5	335650	5	NULL	NULL	0	NULL	statement 3			abolishes					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13856_s_174	10788509	Replacement of sodium by choline abolished glycine induced steady-state currents in wild type and mutant transporters.	transcription
60881	1	335650	7	NULL	NULL	0	NULL	glycine	AminoAcid		induce					transporter	GP	steady-state current;; wild type			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_18_13856_s_174	10788509	Replacement of sodium by choline abolished glycine induced steady-state currents in wild type and mutant transporters.	transcription
60882	2	335650	7	NULL	NULL	0	NULL	glycine	AminoAcid		induce					transporter	GP	steady-state current;;mutant			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_18_13856_s_174	10788509	Replacement of sodium by choline abolished glycine induced steady-state currents in wild type and mutant transporters.	transcription
60883	3	335650	7	NULL	NULL	0	NULL	sodium	Chemical		replaced by					choline	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13856_s_174	10788509	Replacement of sodium by choline abolished glycine induced steady-state currents in wild type and mutant transporters.	transcription
60884	4	335650	7	NULL	NULL	0	NULL	statement 3	Process		abolish					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13856_s_174	10788509	Replacement of sodium by choline abolished glycine induced steady-state currents in wild type and mutant transporters.	transcription
60885	5	335650	7	NULL	NULL	0	NULL	statement 3	Process		abolish					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13856_s_174	10788509	Replacement of sodium by choline abolished glycine induced steady-state currents in wild type and mutant transporters.	transcription
56331	1	335651	5	NULL	NULL	0	NULL	choline- O-sulfate			hydrolyzed to					choline					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_560_s_227	0009925583	Recently, Osteraos et al. ( 50) reported the presence of a choline sulfatase activity (BetC) in the rhizosphere bacterium  Sinorhizobium meliloti that catalyzed the hydrolysis of choline- O-sulfate into choline and sulfate; the produced choline was then further oxidized into glycine betaine by the BetA and BetB enzymes.	transcription
56332	2	335651	5	NULL	NULL	0	NULL	choline- O-sulfate			hydrolyzed to					sulfate					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_560_s_227	0009925583	Recently, Osteraos et al. ( 50) reported the presence of a choline sulfatase activity (BetC) in the rhizosphere bacterium  Sinorhizobium meliloti that catalyzed the hydrolysis of choline- O-sulfate into choline and sulfate; the produced choline was then further oxidized into glycine betaine by the BetA and BetB enzymes.	transcription
56333	3	335651	5	NULL	NULL	0	NULL	statement 1			occurs along with					statement 2					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_560_s_227	0009925583	Recently, Osteraos et al. ( 50) reported the presence of a choline sulfatase activity (BetC) in the rhizosphere bacterium  Sinorhizobium meliloti that catalyzed the hydrolysis of choline- O-sulfate into choline and sulfate; the produced choline was then further oxidized into glycine betaine by the BetA and BetB enzymes.	transcription
56334	4	335651	5	NULL	NULL	0	NULL	BetC		Sinorhizobium meliloti	catalyze					statement 3					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_560_s_227	0009925583	Recently, Osteraos et al. ( 50) reported the presence of a choline sulfatase activity (BetC) in the rhizosphere bacterium  Sinorhizobium meliloti that catalyzed the hydrolysis of choline- O-sulfate into choline and sulfate; the produced choline was then further oxidized into glycine betaine by the BetA and BetB enzymes.	transcription
56335	5	335651	5	NULL	NULL	0	NULL	Sinorhizobium meliloti			is a type of					rhizosphere bacterium					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_560_s_227	0009925583	Recently, Osteraos et al. ( 50) reported the presence of a choline sulfatase activity (BetC) in the rhizosphere bacterium  Sinorhizobium meliloti that catalyzed the hydrolysis of choline- O-sulfate into choline and sulfate; the produced choline was then further oxidized into glycine betaine by the BetA and BetB enzymes.	transcription
56364	6	335651	5	NULL	NULL	0	NULL	choline			is oxidized to					glycine betaine					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_560_s_227	0009925583	Recently, Osteraos et al. ( 50) reported the presence of a choline sulfatase activity (BetC) in the rhizosphere bacterium  Sinorhizobium meliloti that catalyzed the hydrolysis of choline- O-sulfate into choline and sulfate; the produced choline was then further oxidized into glycine betaine by the BetA and BetB enzymes.	transcription
56365	7	335651	5	NULL	NULL	0	NULL	BetA enzyme			catalyzes					statement 6					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_560_s_227	0009925583	Recently, Osteraos et al. ( 50) reported the presence of a choline sulfatase activity (BetC) in the rhizosphere bacterium  Sinorhizobium meliloti that catalyzed the hydrolysis of choline- O-sulfate into choline and sulfate; the produced choline was then further oxidized into glycine betaine by the BetA and BetB enzymes.	transcription
56366	8	335651	5	NULL	NULL	0	NULL	BetB enzyme			catalyzes					statement 6					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_560_s_227	0009925583	Recently, Osteraos et al. ( 50) reported the presence of a choline sulfatase activity (BetC) in the rhizosphere bacterium  Sinorhizobium meliloti that catalyzed the hydrolysis of choline- O-sulfate into choline and sulfate; the produced choline was then further oxidized into glycine betaine by the BetA and BetB enzymes.	transcription
60886	1	335651	7	NULL	NULL	0	NULL	choline- O-sulfate	Chemical		hydrolyzed to					choline	Chemical				NULL	Sinorhizobium meliloti 	NULL	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_560_s_227	0009925583	Recently, Osteraos et al. ( 50) reported the presence of a choline sulfatase activity (BetC) in the rhizosphere bacterium  Sinorhizobium meliloti that catalyzed the hydrolysis of choline- O-sulfate into choline and sulfate; the produced choline was then further oxidized into glycine betaine by the BetA and BetB enzymes.	transcription
60887	2	335651	7	NULL	NULL	0	NULL	choline- O-sulfate	Chemical		hydrolyzed to					sulfate	Chemical				NULL	Sinorhizobium meliloti	NULL	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_560_s_227	0009925583	Recently, Osteraos et al. ( 50) reported the presence of a choline sulfatase activity (BetC) in the rhizosphere bacterium  Sinorhizobium meliloti that catalyzed the hydrolysis of choline- O-sulfate into choline and sulfate; the produced choline was then further oxidized into glycine betaine by the BetA and BetB enzymes.	transcription
60888	3	335651	7	NULL	NULL	0	NULL	statement 1	Process		occur simultaneous with					statement 2	Process				NULL	Sinorhizobium meliloti 	NULL	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_560_s_227	0009925583	Recently, Osteraos et al. ( 50) reported the presence of a choline sulfatase activity (BetC) in the rhizosphere bacterium  Sinorhizobium meliloti that catalyzed the hydrolysis of choline- O-sulfate into choline and sulfate; the produced choline was then further oxidized into glycine betaine by the BetA and BetB enzymes.	transcription
60889	4	335651	7	NULL	NULL	0	NULL	BetC	GP		catalyze					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_560_s_227	0009925583	Recently, Osteraos et al. ( 50) reported the presence of a choline sulfatase activity (BetC) in the rhizosphere bacterium  Sinorhizobium meliloti that catalyzed the hydrolysis of choline- O-sulfate into choline and sulfate; the produced choline was then further oxidized into glycine betaine by the BetA and BetB enzymes.	transcription
60890	5	335651	7	NULL	NULL	0	NULL	BetC	GP		catalyze					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_560_s_227	0009925583	Recently, Osteraos et al. ( 50) reported the presence of a choline sulfatase activity (BetC) in the rhizosphere bacterium  Sinorhizobium meliloti that catalyzed the hydrolysis of choline- O-sulfate into choline and sulfate; the produced choline was then further oxidized into glycine betaine by the BetA and BetB enzymes.	transcription
60891	6	335651	7	NULL	NULL	0	NULL	BetC	GP		is					choline sulfatase	GP				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_560_s_227	0009925583	Recently, Osteraos et al. ( 50) reported the presence of a choline sulfatase activity (BetC) in the rhizosphere bacterium  Sinorhizobium meliloti that catalyzed the hydrolysis of choline- O-sulfate into choline and sulfate; the produced choline was then further oxidized into glycine betaine by the BetA and BetB enzymes.	transcription
60895	7	335651	7	NULL	NULL	0	NULL	choline	Chemical		oxidizes to					glycine betaine	AminoAcid				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_560_s_227	0009925583	Recently, Osteraos et al. ( 50) reported the presence of a choline sulfatase activity (BetC) in the rhizosphere bacterium  Sinorhizobium meliloti that catalyzed the hydrolysis of choline- O-sulfate into choline and sulfate; the produced choline was then further oxidized into glycine betaine by the BetA and BetB enzymes.	transcription
60899	8	335651	7	NULL	NULL	0	NULL	BetA	GP		catalyze					statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_560_s_227	0009925583	Recently, Osteraos et al. ( 50) reported the presence of a choline sulfatase activity (BetC) in the rhizosphere bacterium  Sinorhizobium meliloti that catalyzed the hydrolysis of choline- O-sulfate into choline and sulfate; the produced choline was then further oxidized into glycine betaine by the BetA and BetB enzymes.	transcription
60902	9	335651	7	NULL	NULL	0	NULL	BetB	GP		catalyze					statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_560_s_227	0009925583	Recently, Osteraos et al. ( 50) reported the presence of a choline sulfatase activity (BetC) in the rhizosphere bacterium  Sinorhizobium meliloti that catalyzed the hydrolysis of choline- O-sulfate into choline and sulfate; the produced choline was then further oxidized into glycine betaine by the BetA and BetB enzymes.	transcription
60905	10	335651	7	NULL	NULL	0	NULL	Sinorhizobium meliloti	Organism		is a type of					rhizosphere bacterium	Organism				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_560_s_227	0009925583	Recently, Osteraos et al. ( 50) reported the presence of a choline sulfatase activity (BetC) in the rhizosphere bacterium  Sinorhizobium meliloti that catalyzed the hydrolysis of choline- O-sulfate into choline and sulfate; the produced choline was then further oxidized into glycine betaine by the BetA and BetB enzymes.	transcription
56367	1	335652	5	NULL	NULL	0	NULL	choline transport system		A. halophytica	has affinity for		low			choline					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1621_1_102_s_186	12667616	The data in  Fig. 3B revealed that the choline transport system of  A. halophytica had a low affinity for choline ( Km, 272  M) which is in contrast to a rather high affinity for glycine betaine transporter  ( Km, 2  M) [ 15].	transcription
56368	2	335652	5	NULL	NULL	0	NULL	glycine betaine transporter		A. halophytica	has affinity for		high			choline					NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1621_1_102_s_186	12667616	The data in  Fig. 3B revealed that the choline transport system of  A. halophytica had a low affinity for choline ( Km, 272  M) which is in contrast to a rather high affinity for glycine betaine transporter  ( Km, 2  M) [ 15].	transcription
60906	1	335652	7	NULL	NULL	0	NULL	choline transport system	GP	A. halophytica	has low affinity for					choline	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1621_1_102_s_186	12667616	The data in  Fig. 3B revealed that the choline transport system of  A. halophytica had a low affinity for choline ( Km, 272  M) which is in contrast to a rather high affinity for glycine betaine transporter  ( Km, 2  M) [ 15].	transcription
60907	2	335652	7	NULL	NULL	0	NULL	glycine betaine transporter	GP	A. halophytica	high affinity for					choline	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1621_1_102_s_186	12667616	The data in  Fig. 3B revealed that the choline transport system of  A. halophytica had a low affinity for choline ( Km, 272  M) which is in contrast to a rather high affinity for glycine betaine transporter  ( Km, 2  M) [ 15].	transcription
56369	1	335653	5	NULL	NULL	0	NULL	choline			is oxidized to					glycine-betaine					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_32	12676692	Choline dehydrogenase catalyzes the four-electron oxidation of choline to glycine-betaine via a betaine-aldehyde intermediate ( ) (Fig.  1) and shows an absolute requirement for an electron acceptor other than molecular oxygen for catalysis ( ,  ).	transcription
56370	2	335653	5	NULL	NULL	0	NULL	statement 1			via					betaine-aldehyde intermediate					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_32	12676692	Choline dehydrogenase catalyzes the four-electron oxidation of choline to glycine-betaine via a betaine-aldehyde intermediate ( ) (Fig.  1) and shows an absolute requirement for an electron acceptor other than molecular oxygen for catalysis ( ,  ).	transcription
56371	3	335653	5	NULL	NULL	0	NULL	choline dehydrogenase			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_32	12676692	Choline dehydrogenase catalyzes the four-electron oxidation of choline to glycine-betaine via a betaine-aldehyde intermediate ( ) (Fig.  1) and shows an absolute requirement for an electron acceptor other than molecular oxygen for catalysis ( ,  ).	transcription
56372	4	335653	5	NULL	NULL	0	NULL	electron acceptor			is required for					statement 3					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_32	12676692	Choline dehydrogenase catalyzes the four-electron oxidation of choline to glycine-betaine via a betaine-aldehyde intermediate ( ) (Fig.  1) and shows an absolute requirement for an electron acceptor other than molecular oxygen for catalysis ( ,  ).	transcription
60908	1	335653	7	NULL	NULL	0	NULL	choline	Chemical		oxidizes to					glycine-betaine	AminoAcid				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_32	12676692	Choline dehydrogenase catalyzes the four-electron oxidation of choline to glycine-betaine via a betaine-aldehyde intermediate ( ) (Fig.  1) and shows an absolute requirement for an electron acceptor other than molecular oxygen for catalysis ( ,  ).	transcription
60909	2	335653	7	NULL	NULL	0	NULL	statement 1	Process		via					betaine-aldehyde intermediate	Chemical				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_32	12676692	Choline dehydrogenase catalyzes the four-electron oxidation of choline to glycine-betaine via a betaine-aldehyde intermediate ( ) (Fig.  1) and shows an absolute requirement for an electron acceptor other than molecular oxygen for catalysis ( ,  ).	transcription
60910	3	335653	7	NULL	NULL	0	NULL	Choline dehydrogenase	GP		catalyze					statement 1	Process	four-electron oxidation of			NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_32	12676692	Choline dehydrogenase catalyzes the four-electron oxidation of choline to glycine-betaine via a betaine-aldehyde intermediate ( ) (Fig.  1) and shows an absolute requirement for an electron acceptor other than molecular oxygen for catalysis ( ,  ).	transcription
60914	4	335653	7	NULL	NULL	0	NULL	statement 3	Process		require					electron acceptor	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_32	12676692	Choline dehydrogenase catalyzes the four-electron oxidation of choline to glycine-betaine via a betaine-aldehyde intermediate ( ) (Fig.  1) and shows an absolute requirement for an electron acceptor other than molecular oxygen for catalysis ( ,  ).	transcription
60918	5	335653	7	NULL	NULL	0	NULL	statement 3	Process		require					molecular oxygen	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_32	12676692	Choline dehydrogenase catalyzes the four-electron oxidation of choline to glycine-betaine via a betaine-aldehyde intermediate ( ) (Fig.  1) and shows an absolute requirement for an electron acceptor other than molecular oxygen for catalysis ( ,  ).	transcription
56373	1	335654	5	NULL	NULL	0	NULL	glycine-betaine			is produced from					choline					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_24	12676692	In  E. coli, the biosynthetic pathway for the production of glycine-betaine from choline has been well characterized at the genetic level, where it has been shown that four genes encoding choline dehydrogenase ( betA), betaine-aldehyde dehydrogenase ( betB), a putative regulator ( betI), and a choline transporter ( betT) are clustered in the  bet operon ( ).	transcription
56374	2	335654	5	NULL	NULL	0	NULL	betA gene			clustered in									bet operon	NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_24	12676692	In  E. coli, the biosynthetic pathway for the production of glycine-betaine from choline has been well characterized at the genetic level, where it has been shown that four genes encoding choline dehydrogenase ( betA), betaine-aldehyde dehydrogenase ( betB), a putative regulator ( betI), and a choline transporter ( betT) are clustered in the  bet operon ( ).	transcription
56375	3	335654	5	NULL	NULL	0	NULL	betB gene			clustered in									bet operon	NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_24	12676692	In  E. coli, the biosynthetic pathway for the production of glycine-betaine from choline has been well characterized at the genetic level, where it has been shown that four genes encoding choline dehydrogenase ( betA), betaine-aldehyde dehydrogenase ( betB), a putative regulator ( betI), and a choline transporter ( betT) are clustered in the  bet operon ( ).	transcription
56376	4	335654	5	NULL	NULL	0	NULL	betI gene			clustered in									bet operon	NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_24	12676692	In  E. coli, the biosynthetic pathway for the production of glycine-betaine from choline has been well characterized at the genetic level, where it has been shown that four genes encoding choline dehydrogenase ( betA), betaine-aldehyde dehydrogenase ( betB), a putative regulator ( betI), and a choline transporter ( betT) are clustered in the  bet operon ( ).	transcription
56377	5	335654	5	NULL	NULL	0	NULL	betT gene			clustered in									bet operon	NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_24	12676692	In  E. coli, the biosynthetic pathway for the production of glycine-betaine from choline has been well characterized at the genetic level, where it has been shown that four genes encoding choline dehydrogenase ( betA), betaine-aldehyde dehydrogenase ( betB), a putative regulator ( betI), and a choline transporter ( betT) are clustered in the  bet operon ( ).	transcription
56378	6	335654	5	NULL	NULL	0	NULL	statement 2			occurs simultaneously with					statement 3					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_24	12676692	In  E. coli, the biosynthetic pathway for the production of glycine-betaine from choline has been well characterized at the genetic level, where it has been shown that four genes encoding choline dehydrogenase ( betA), betaine-aldehyde dehydrogenase ( betB), a putative regulator ( betI), and a choline transporter ( betT) are clustered in the  bet operon ( ).	transcription
56379	7	335654	5	NULL	NULL	0	NULL	statement 4			occurs simultaneously with					statement 5					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_24	12676692	In  E. coli, the biosynthetic pathway for the production of glycine-betaine from choline has been well characterized at the genetic level, where it has been shown that four genes encoding choline dehydrogenase ( betA), betaine-aldehyde dehydrogenase ( betB), a putative regulator ( betI), and a choline transporter ( betT) are clustered in the  bet operon ( ).	transcription
56380	8	335654	5	NULL	NULL	0	NULL	betA gene			encodes					choline dehydrogenase					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_24	12676692	In  E. coli, the biosynthetic pathway for the production of glycine-betaine from choline has been well characterized at the genetic level, where it has been shown that four genes encoding choline dehydrogenase ( betA), betaine-aldehyde dehydrogenase ( betB), a putative regulator ( betI), and a choline transporter ( betT) are clustered in the  bet operon ( ).	transcription
56381	9	335654	5	NULL	NULL	0	NULL	betB gene			encodes					betaine-aldehyde dehydrogenase					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_24	12676692	In  E. coli, the biosynthetic pathway for the production of glycine-betaine from choline has been well characterized at the genetic level, where it has been shown that four genes encoding choline dehydrogenase ( betA), betaine-aldehyde dehydrogenase ( betB), a putative regulator ( betI), and a choline transporter ( betT) are clustered in the  bet operon ( ).	transcription
56382	10	335654	5	NULL	NULL	0	NULL	betI gene			is a type of					putative regulator					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_24	12676692	In  E. coli, the biosynthetic pathway for the production of glycine-betaine from choline has been well characterized at the genetic level, where it has been shown that four genes encoding choline dehydrogenase ( betA), betaine-aldehyde dehydrogenase ( betB), a putative regulator ( betI), and a choline transporter ( betT) are clustered in the  bet operon ( ).	transcription
56383	11	335654	5	NULL	NULL	0	NULL	betT gene			encodes					choline transporter					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_24	12676692	In  E. coli, the biosynthetic pathway for the production of glycine-betaine from choline has been well characterized at the genetic level, where it has been shown that four genes encoding choline dehydrogenase ( betA), betaine-aldehyde dehydrogenase ( betB), a putative regulator ( betI), and a choline transporter ( betT) are clustered in the  bet operon ( ).	transcription
60920	1	335654	7	NULL	NULL	0	NULL	glycine-betaine	AminoAcid		produced from					choline	Chemical				NULL	E.coli	0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_24	12676692	In  E. coli, the biosynthetic pathway for the production of glycine-betaine from choline has been well characterized at the genetic level, where it has been shown that four genes encoding choline dehydrogenase ( betA), betaine-aldehyde dehydrogenase ( betB), a putative regulator ( betI), and a choline transporter ( betT) are clustered in the  bet operon ( ).	transcription
60921	2	335654	7	NULL	NULL	0	NULL	betA	GP		encode					choline dehydrogenase	GP				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_24	12676692	In  E. coli, the biosynthetic pathway for the production of glycine-betaine from choline has been well characterized at the genetic level, where it has been shown that four genes encoding choline dehydrogenase ( betA), betaine-aldehyde dehydrogenase ( betB), a putative regulator ( betI), and a choline transporter ( betT) are clustered in the  bet operon ( ).	transcription
60922	3	335654	7	NULL	NULL	0	NULL	 betB	GP		encode					betaine-aldehyde dehydrogenase	GP				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_24	12676692	In  E. coli, the biosynthetic pathway for the production of glycine-betaine from choline has been well characterized at the genetic level, where it has been shown that four genes encoding choline dehydrogenase ( betA), betaine-aldehyde dehydrogenase ( betB), a putative regulator ( betI), and a choline transporter ( betT) are clustered in the  bet operon ( ).	transcription
60923	4	335654	7	NULL	NULL	0	NULL	betI	GP		encode					putative regulator	GP				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_24	12676692	In  E. coli, the biosynthetic pathway for the production of glycine-betaine from choline has been well characterized at the genetic level, where it has been shown that four genes encoding choline dehydrogenase ( betA), betaine-aldehyde dehydrogenase ( betB), a putative regulator ( betI), and a choline transporter ( betT) are clustered in the  bet operon ( ).	transcription
60924	5	335654	7	NULL	NULL	0	NULL	betT	GP		encode					choline transporter	GP				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_24	12676692	In  E. coli, the biosynthetic pathway for the production of glycine-betaine from choline has been well characterized at the genetic level, where it has been shown that four genes encoding choline dehydrogenase ( betA), betaine-aldehyde dehydrogenase ( betB), a putative regulator ( betI), and a choline transporter ( betT) are clustered in the  bet operon ( ).	transcription
60925	6	335654	7	NULL	NULL	0	NULL	betA	GP		clustered in					bet operon	GP				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_24	12676692	In  E. coli, the biosynthetic pathway for the production of glycine-betaine from choline has been well characterized at the genetic level, where it has been shown that four genes encoding choline dehydrogenase ( betA), betaine-aldehyde dehydrogenase ( betB), a putative regulator ( betI), and a choline transporter ( betT) are clustered in the  bet operon ( ).	transcription
60926	7	335654	7	NULL	NULL	0	NULL	betB	GP		clustered in					bet operon	GP				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_24	12676692	In  E. coli, the biosynthetic pathway for the production of glycine-betaine from choline has been well characterized at the genetic level, where it has been shown that four genes encoding choline dehydrogenase ( betA), betaine-aldehyde dehydrogenase ( betB), a putative regulator ( betI), and a choline transporter ( betT) are clustered in the  bet operon ( ).	transcription
60927	8	335654	7	NULL	NULL	0	NULL	betI	GP		clustered in					bet operon	GP				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_24	12676692	In  E. coli, the biosynthetic pathway for the production of glycine-betaine from choline has been well characterized at the genetic level, where it has been shown that four genes encoding choline dehydrogenase ( betA), betaine-aldehyde dehydrogenase ( betB), a putative regulator ( betI), and a choline transporter ( betT) are clustered in the  bet operon ( ).	transcription
60928	9	335654	7	NULL	NULL	0	NULL	betT	GP		clustered in					bet operon	GP				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_4_2126_s_24	12676692	In  E. coli, the biosynthetic pathway for the production of glycine-betaine from choline has been well characterized at the genetic level, where it has been shown that four genes encoding choline dehydrogenase ( betA), betaine-aldehyde dehydrogenase ( betB), a putative regulator ( betI), and a choline transporter ( betT) are clustered in the  bet operon ( ).	transcription
56384	1	335655	5	NULL	NULL	0	NULL	choline		uptake of	occurs by					transport activity		constitutive low-affinity			NULL	R. meliloti	0	NULL	NULL	NULL	gw70_annurevmicrobiol_50_0_101_s_272	8905077	However, Pocard et al ( 111) also showed that glycine betaine is not a potent inhibitor of choline uptake by  the constitutive low-affinity transport activity of  R. meliloti.	transcription
56385	2	335655	5	NULL	NULL	0	NULL	glycine betaine			is not an inhibitor of		potent			statement 1					NULL	R. meliloti	0	NULL	NULL	NULL	gw70_annurevmicrobiol_50_0_101_s_272	8905077	However, Pocard et al ( 111) also showed that glycine betaine is not a potent inhibitor of choline uptake by  the constitutive low-affinity transport activity of  R. meliloti.	transcription
60929	1	335655	7	NULL	NULL	0	NULL	glycine betaine	AminoAcid		is not potent inhibitor of					choline	Chemical	uptake of			NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_50_0_101_s_272	8905077	However, Pocard et al ( 111) also showed that glycine betaine is not a potent inhibitor of choline uptake by  the constitutive low-affinity transport activity of  R. meliloti.	transcription
60930	2	335655	7	NULL	NULL	0	NULL	R. meliloti	Organism		possess					transport activity	Process	 constitutive low-affinity 			NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_50_0_101_s_272	8905077	However, Pocard et al ( 111) also showed that glycine betaine is not a potent inhibitor of choline uptake by  the constitutive low-affinity transport activity of  R. meliloti.	transcription
56386	1	335656	5	NULL	NULL	0	NULL	alanine			reduce		slightly			GABA		rates of;;transport of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_11_7197_s_115	16407306	Alanine slightly reduced GABA transport rates, whereas histidine as well as compounds that were good competitors for ProT-mediated GABA transport ( i.e.D- and L-proline, glycine betaine, and choline) did not reduce GABA uptake activity ( ).	transcription
56387	2	335656	5	NULL	NULL	0	NULL	histidine			does not reduce					GABA		uptake of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_11_7197_s_115	16407306	Alanine slightly reduced GABA transport rates, whereas histidine as well as compounds that were good competitors for ProT-mediated GABA transport ( i.e.D- and L-proline, glycine betaine, and choline) did not reduce GABA uptake activity ( ).	transcription
56388	3	335656	5	NULL	NULL	0	NULL	D-proline			does not reduce					GABA		uptake of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_11_7197_s_115	16407306	Alanine slightly reduced GABA transport rates, whereas histidine as well as compounds that were good competitors for ProT-mediated GABA transport ( i.e.D- and L-proline, glycine betaine, and choline) did not reduce GABA uptake activity ( ).	transcription
56389	4	335656	5	NULL	NULL	0	NULL	L-proline			does not reduce					GABA		uptake of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_11_7197_s_115	16407306	Alanine slightly reduced GABA transport rates, whereas histidine as well as compounds that were good competitors for ProT-mediated GABA transport ( i.e.D- and L-proline, glycine betaine, and choline) did not reduce GABA uptake activity ( ).	transcription
56390	5	335656	5	NULL	NULL	0	NULL	glycine betaine			does not reduce					GABA		uptake of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_11_7197_s_115	16407306	Alanine slightly reduced GABA transport rates, whereas histidine as well as compounds that were good competitors for ProT-mediated GABA transport ( i.e.D- and L-proline, glycine betaine, and choline) did not reduce GABA uptake activity ( ).	transcription
56391	6	335656	5	NULL	NULL	0	NULL	choline			does not reduce					GABA		uptake of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_11_7197_s_115	16407306	Alanine slightly reduced GABA transport rates, whereas histidine as well as compounds that were good competitors for ProT-mediated GABA transport ( i.e.D- and L-proline, glycine betaine, and choline) did not reduce GABA uptake activity ( ).	transcription
56392	7	335656	5	NULL	NULL	0	NULL	ProT			mediate					GABA		transport of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_11_7197_s_115	16407306	Alanine slightly reduced GABA transport rates, whereas histidine as well as compounds that were good competitors for ProT-mediated GABA transport ( i.e.D- and L-proline, glycine betaine, and choline) did not reduce GABA uptake activity ( ).	transcription
56393	8	335656	5	NULL	NULL	0	NULL	histidine			mediate					GABA		transport of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_11_7197_s_115	16407306	Alanine slightly reduced GABA transport rates, whereas histidine as well as compounds that were good competitors for ProT-mediated GABA transport ( i.e.D- and L-proline, glycine betaine, and choline) did not reduce GABA uptake activity ( ).	transcription
56394	9	335656	5	NULL	NULL	0	NULL	statement 8			competes with					statement 7					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_11_7197_s_115	16407306	Alanine slightly reduced GABA transport rates, whereas histidine as well as compounds that were good competitors for ProT-mediated GABA transport ( i.e.D- and L-proline, glycine betaine, and choline) did not reduce GABA uptake activity ( ).	transcription
56395	10	335656	5	NULL	NULL	0	NULL	D-proline			mediate					GABA		transport of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_11_7197_s_115	16407306	Alanine slightly reduced GABA transport rates, whereas histidine as well as compounds that were good competitors for ProT-mediated GABA transport ( i.e.D- and L-proline, glycine betaine, and choline) did not reduce GABA uptake activity ( ).	transcription
56396	11	335656	5	NULL	NULL	0	NULL	statement 10			competes with					statement 7					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_11_7197_s_115	16407306	Alanine slightly reduced GABA transport rates, whereas histidine as well as compounds that were good competitors for ProT-mediated GABA transport ( i.e.D- and L-proline, glycine betaine, and choline) did not reduce GABA uptake activity ( ).	transcription
56397	12	335656	5	NULL	NULL	0	NULL	L-proline			mediate					GABA		transport of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_11_7197_s_115	16407306	Alanine slightly reduced GABA transport rates, whereas histidine as well as compounds that were good competitors for ProT-mediated GABA transport ( i.e.D- and L-proline, glycine betaine, and choline) did not reduce GABA uptake activity ( ).	transcription
56398	13	335656	5	NULL	NULL	0	NULL	statement 12			competes with					statement 7					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_11_7197_s_115	16407306	Alanine slightly reduced GABA transport rates, whereas histidine as well as compounds that were good competitors for ProT-mediated GABA transport ( i.e.D- and L-proline, glycine betaine, and choline) did not reduce GABA uptake activity ( ).	transcription
56399	14	335656	5	NULL	NULL	0	NULL	glycine betaine			mediate					GABA		transport of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_11_7197_s_115	16407306	Alanine slightly reduced GABA transport rates, whereas histidine as well as compounds that were good competitors for ProT-mediated GABA transport ( i.e.D- and L-proline, glycine betaine, and choline) did not reduce GABA uptake activity ( ).	transcription
56400	15	335656	5	NULL	NULL	0	NULL	statement 14			competes with					statement 7					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_11_7197_s_115	16407306	Alanine slightly reduced GABA transport rates, whereas histidine as well as compounds that were good competitors for ProT-mediated GABA transport ( i.e.D- and L-proline, glycine betaine, and choline) did not reduce GABA uptake activity ( ).	transcription
56401	16	335656	5	NULL	NULL	0	NULL	choline			mediate					GABA		transport of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_11_7197_s_115	16407306	Alanine slightly reduced GABA transport rates, whereas histidine as well as compounds that were good competitors for ProT-mediated GABA transport ( i.e.D- and L-proline, glycine betaine, and choline) did not reduce GABA uptake activity ( ).	transcription
56402	17	335656	5	NULL	NULL	0	NULL	statement 16			competes with					statement 7					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_11_7197_s_115	16407306	Alanine slightly reduced GABA transport rates, whereas histidine as well as compounds that were good competitors for ProT-mediated GABA transport ( i.e.D- and L-proline, glycine betaine, and choline) did not reduce GABA uptake activity ( ).	transcription
60931	1	335656	7	NULL	NULL	0	NULL	Alanine	AminoAcid		reduce		slightly			GABA 	Process	rate of transport of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_11_7197_s_115	16407306	Alanine slightly reduced GABA transport rates, whereas histidine as well as compounds that were good competitors for ProT-mediated GABA transport ( i.e.D- and L-proline, glycine betaine, and choline) did not reduce GABA uptake activity ( ).	transcription
60932	2	335656	7	NULL	NULL	0	NULL	ProT	GP		mediate					GABA 	Process	transport of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_11_7197_s_115	16407306	Alanine slightly reduced GABA transport rates, whereas histidine as well as compounds that were good competitors for ProT-mediated GABA transport ( i.e.D- and L-proline, glycine betaine, and choline) did not reduce GABA uptake activity ( ).	transcription
60933	3	335656	7	NULL	NULL	0	NULL	histidine 	AminoAcid		compete with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_11_7197_s_115	16407306	Alanine slightly reduced GABA transport rates, whereas histidine as well as compounds that were good competitors for ProT-mediated GABA transport ( i.e.D- and L-proline, glycine betaine, and choline) did not reduce GABA uptake activity ( ).	transcription
60934	4	335656	7	NULL	NULL	0	NULL	D-proline	AminoAcid		does not reduce					GABA	Chemical	uptake activity of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_11_7197_s_115	16407306	Alanine slightly reduced GABA transport rates, whereas histidine as well as compounds that were good competitors for ProT-mediated GABA transport ( i.e.D- and L-proline, glycine betaine, and choline) did not reduce GABA uptake activity ( ).	transcription
60935	5	335656	7	NULL	NULL	0	NULL	L-proline	AminoAcid		does not reduce					GABA	Chemical	uptake activity of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_11_7197_s_115	16407306	Alanine slightly reduced GABA transport rates, whereas histidine as well as compounds that were good competitors for ProT-mediated GABA transport ( i.e.D- and L-proline, glycine betaine, and choline) did not reduce GABA uptake activity ( ).	transcription
60936	6	335656	7	NULL	NULL	0	NULL	glycine betaine	AminoAcid		does not reduce					GABA	Chemical	uptake activity of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_11_7197_s_115	16407306	Alanine slightly reduced GABA transport rates, whereas histidine as well as compounds that were good competitors for ProT-mediated GABA transport ( i.e.D- and L-proline, glycine betaine, and choline) did not reduce GABA uptake activity ( ).	transcription
60937	7	335656	7	NULL	NULL	0	NULL	choline	Chemical		does not reduce					GABA 	Chemical	uptake activity of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_11_7197_s_115	16407306	Alanine slightly reduced GABA transport rates, whereas histidine as well as compounds that were good competitors for ProT-mediated GABA transport ( i.e.D- and L-proline, glycine betaine, and choline) did not reduce GABA uptake activity ( ).	transcription
56403	1	335657	5	NULL	NULL	0	NULL	glycine betaine			inhibits		strongly			GABA		transport of			NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_99	10359089	Glycine betaine and its immediate metabolic precursors, betaine aldehyde and choline, were strong inhibitors; other betaines, including carnitine, trigonelline and betonicine, also inhibited GABA transport, but were not as effective.	transcription
56404	2	335657	5	NULL	NULL	0	NULL	betaine aldehyde			inhibits		strongly			GABA		transport of			NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_99	10359089	Glycine betaine and its immediate metabolic precursors, betaine aldehyde and choline, were strong inhibitors; other betaines, including carnitine, trigonelline and betonicine, also inhibited GABA transport, but were not as effective.	transcription
56405	3	335657	5	NULL	NULL	0	NULL	choline			inhibits		strongly			GABA		transport of			NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_99	10359089	Glycine betaine and its immediate metabolic precursors, betaine aldehyde and choline, were strong inhibitors; other betaines, including carnitine, trigonelline and betonicine, also inhibited GABA transport, but were not as effective.	transcription
56406	4	335657	5	NULL	NULL	0	NULL	betaine aldehyde			is a metabolic precursor of					glycine betaine					NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_99	10359089	Glycine betaine and its immediate metabolic precursors, betaine aldehyde and choline, were strong inhibitors; other betaines, including carnitine, trigonelline and betonicine, also inhibited GABA transport, but were not as effective.	transcription
56407	5	335657	5	NULL	NULL	0	NULL	choline			is a metabolic precursor of					glycine betaine					NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_99	10359089	Glycine betaine and its immediate metabolic precursors, betaine aldehyde and choline, were strong inhibitors; other betaines, including carnitine, trigonelline and betonicine, also inhibited GABA transport, but were not as effective.	transcription
56408	6	335657	5	NULL	NULL	0	NULL	carnitine			is a type of					betaines					NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_99	10359089	Glycine betaine and its immediate metabolic precursors, betaine aldehyde and choline, were strong inhibitors; other betaines, including carnitine, trigonelline and betonicine, also inhibited GABA transport, but were not as effective.	transcription
56409	7	335657	5	NULL	NULL	0	NULL	trigonelline			is a type of					betaines					NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_99	10359089	Glycine betaine and its immediate metabolic precursors, betaine aldehyde and choline, were strong inhibitors; other betaines, including carnitine, trigonelline and betonicine, also inhibited GABA transport, but were not as effective.	transcription
56410	8	335657	5	NULL	NULL	0	NULL	betonicine			is a type of					betaines					NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_99	10359089	Glycine betaine and its immediate metabolic precursors, betaine aldehyde and choline, were strong inhibitors; other betaines, including carnitine, trigonelline and betonicine, also inhibited GABA transport, but were not as effective.	transcription
56411	9	335657	5	NULL	NULL	0	NULL	carnitine			inhibits					GABA		transport of			NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_99	10359089	Glycine betaine and its immediate metabolic precursors, betaine aldehyde and choline, were strong inhibitors; other betaines, including carnitine, trigonelline and betonicine, also inhibited GABA transport, but were not as effective.	transcription
56412	10	335657	5	NULL	NULL	0	NULL	trigonelline			inhibits					GABA		transport of			NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_99	10359089	Glycine betaine and its immediate metabolic precursors, betaine aldehyde and choline, were strong inhibitors; other betaines, including carnitine, trigonelline and betonicine, also inhibited GABA transport, but were not as effective.	transcription
56413	11	335657	5	NULL	NULL	0	NULL	betonicine			inhibits					GABA		transport of			NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_99	10359089	Glycine betaine and its immediate metabolic precursors, betaine aldehyde and choline, were strong inhibitors; other betaines, including carnitine, trigonelline and betonicine, also inhibited GABA transport, but were not as effective.	transcription
60938	1	335657	7	NULL	NULL	0	NULL	Glycine betaine	AminoAcid		inhibit		strongly			GABA	Chemical	transport of			NULL		NULL	NULL	NULL	NULL	gw60_febslett_450_3_280_s_99	10359089	Glycine betaine and its immediate metabolic precursors, betaine aldehyde and choline, were strong inhibitors; other betaines, including carnitine, trigonelline and betonicine, also inhibited GABA transport, but were not as effective.	transcription
60939	2	335657	7	NULL	NULL	0	NULL	betaine aldehyde	Chemical		inhibit		strongly			GABA	Chemical	transport of			NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_99	10359089	Glycine betaine and its immediate metabolic precursors, betaine aldehyde and choline, were strong inhibitors; other betaines, including carnitine, trigonelline and betonicine, also inhibited GABA transport, but were not as effective.	transcription
60940	3	335657	7	NULL	NULL	0	NULL	choline	Chemical		inhibit		strongly			GABA	Chemical	transport of			NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_99	10359089	Glycine betaine and its immediate metabolic precursors, betaine aldehyde and choline, were strong inhibitors; other betaines, including carnitine, trigonelline and betonicine, also inhibited GABA transport, but were not as effective.	transcription
60941	4	335657	7	NULL	NULL	0	NULL	carnitine	Chemical		inhibit					GABA	Chemical	transport of			NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_99	10359089	Glycine betaine and its immediate metabolic precursors, betaine aldehyde and choline, were strong inhibitors; other betaines, including carnitine, trigonelline and betonicine, also inhibited GABA transport, but were not as effective.	transcription
60942	5	335657	7	NULL	NULL	0	NULL	 trigonelline	Chemical		inhibit					GABA	Chemical	transport of			NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_99	10359089	Glycine betaine and its immediate metabolic precursors, betaine aldehyde and choline, were strong inhibitors; other betaines, including carnitine, trigonelline and betonicine, also inhibited GABA transport, but were not as effective.	transcription
60943	6	335657	7	NULL	NULL	0	NULL	betonicine	Chemical		inhibit					GABA	Chemical	transport of			NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_99	10359089	Glycine betaine and its immediate metabolic precursors, betaine aldehyde and choline, were strong inhibitors; other betaines, including carnitine, trigonelline and betonicine, also inhibited GABA transport, but were not as effective.	transcription
60944	7	335657	7	NULL	NULL	0	NULL	statement 4	Process		is not as effective as					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_99	10359089	Glycine betaine and its immediate metabolic precursors, betaine aldehyde and choline, were strong inhibitors; other betaines, including carnitine, trigonelline and betonicine, also inhibited GABA transport, but were not as effective.	transcription
60945	8	335657	7	NULL	NULL	0	NULL	statement 4	Process		is not as effective as					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_99	10359089	Glycine betaine and its immediate metabolic precursors, betaine aldehyde and choline, were strong inhibitors; other betaines, including carnitine, trigonelline and betonicine, also inhibited GABA transport, but were not as effective.	transcription
60946	9	335657	7	NULL	NULL	0	NULL	statement 4	Process		is not as effective as					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_99	10359089	Glycine betaine and its immediate metabolic precursors, betaine aldehyde and choline, were strong inhibitors; other betaines, including carnitine, trigonelline and betonicine, also inhibited GABA transport, but were not as effective.	transcription
60947	10	335657	7	NULL	NULL	0	NULL	statement 5	Process		is not as effective as					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_99	10359089	Glycine betaine and its immediate metabolic precursors, betaine aldehyde and choline, were strong inhibitors; other betaines, including carnitine, trigonelline and betonicine, also inhibited GABA transport, but were not as effective.	transcription
60948	11	335657	7	NULL	NULL	0	NULL	statement 5	Process		is not as effective as					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_99	10359089	Glycine betaine and its immediate metabolic precursors, betaine aldehyde and choline, were strong inhibitors; other betaines, including carnitine, trigonelline and betonicine, also inhibited GABA transport, but were not as effective.	transcription
60949	12	335657	7	NULL	NULL	0	NULL	statement 5	Process		is not as effective as					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_99	10359089	Glycine betaine and its immediate metabolic precursors, betaine aldehyde and choline, were strong inhibitors; other betaines, including carnitine, trigonelline and betonicine, also inhibited GABA transport, but were not as effective.	transcription
60950	13	335657	7	NULL	NULL	0	NULL	statement 6	Process		is not as effective as					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_99	10359089	Glycine betaine and its immediate metabolic precursors, betaine aldehyde and choline, were strong inhibitors; other betaines, including carnitine, trigonelline and betonicine, also inhibited GABA transport, but were not as effective.	transcription
60951	14	335657	7	NULL	NULL	0	NULL	statement 6	Process		is not as effective as					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_99	10359089	Glycine betaine and its immediate metabolic precursors, betaine aldehyde and choline, were strong inhibitors; other betaines, including carnitine, trigonelline and betonicine, also inhibited GABA transport, but were not as effective.	transcription
60952	15	335657	7	NULL	NULL	0	NULL	statement 6	Process		is not as effective as					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_99	10359089	Glycine betaine and its immediate metabolic precursors, betaine aldehyde and choline, were strong inhibitors; other betaines, including carnitine, trigonelline and betonicine, also inhibited GABA transport, but were not as effective.	transcription
60953	16	335657	7	NULL	NULL	0	NULL	carnitine	Chemical		is a type of					betaine	Chemical				NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_99	10359089	Glycine betaine and its immediate metabolic precursors, betaine aldehyde and choline, were strong inhibitors; other betaines, including carnitine, trigonelline and betonicine, also inhibited GABA transport, but were not as effective.	transcription
60954	17	335657	7	NULL	NULL	0	NULL	trigonelline	Chemical		is a type of					betaine	Chemical				NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_99	10359089	Glycine betaine and its immediate metabolic precursors, betaine aldehyde and choline, were strong inhibitors; other betaines, including carnitine, trigonelline and betonicine, also inhibited GABA transport, but were not as effective.	transcription
60955	18	335657	7	NULL	NULL	0	NULL	betonicine	Chemical		is a type of					betaine	Chemical				NULL		0	NULL	NULL	NULL	gw60_febslett_450_3_280_s_99	10359089	Glycine betaine and its immediate metabolic precursors, betaine aldehyde and choline, were strong inhibitors; other betaines, including carnitine, trigonelline and betonicine, also inhibited GABA transport, but were not as effective.	transcription
56414	1	335658	5	NULL	NULL	0	NULL	glycine betaine			stimulates					E.coli		growth of			NULL	hypertonic media	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1420_1_30_s_335	10446288	Glycine betaine, choline and other urine constituents with dietary origins (e.g. proline betaine) stimulate growth of  E. coli, the primary causative agent of ascending urinary tract infections, in hypertonic media [  46].	transcription
56415	2	335658	5	NULL	NULL	0	NULL	choline			stimulates					E.coli		growth of			NULL	hypertonic media	0	NULL	NULL	NULL	gw60_biochimbiophysacta_1420_1_30_s_335	10446288	Glycine betaine, choline and other urine constituents with dietary origins (e.g. proline betaine) stimulate growth of  E. coli, the primary causative agent of ascending urinary tract infections, in hypertonic media [  46].	transcription
56416	3	335658	5	NULL	NULL	0	NULL	proline betaine			stimulates					E.coli		growth of			NULL	hypertonic media	0	NULL	NULL	NULL	gw60_biochimbiophysacta_1420_1_30_s_335	10446288	Glycine betaine, choline and other urine constituents with dietary origins (e.g. proline betaine) stimulate growth of  E. coli, the primary causative agent of ascending urinary tract infections, in hypertonic media [  46].	transcription
56417	4	335658	5	NULL	NULL	0	NULL	E. coli			is causative agent of		primary			ascending urinary tract infections					NULL	hypertonic media	0	NULL	NULL	NULL	gw60_biochimbiophysacta_1420_1_30_s_335	10446288	Glycine betaine, choline and other urine constituents with dietary origins (e.g. proline betaine) stimulate growth of  E. coli, the primary causative agent of ascending urinary tract infections, in hypertonic media [  46].	transcription
60956	1	335658	7	NULL	NULL	0	NULL	Glycine betaine	AminoAcid		stimulate					E.coli	Organism	growth of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1420_1_30_s_335	10446288	Glycine betaine, choline and other urine constituents with dietary origins (e.g. proline betaine) stimulate growth of  E. coli, the primary causative agent of ascending urinary tract infections, in hypertonic media [  46].	transcription
60957	2	335658	7	NULL	NULL	0	NULL	choline	chemical		stimulate					E.coli	Organism	growth of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1420_1_30_s_335	10446288	Glycine betaine, choline and other urine constituents with dietary origins (e.g. proline betaine) stimulate growth of  E. coli, the primary causative agent of ascending urinary tract infections, in hypertonic media [  46].	transcription
60958	3	335658	7	NULL	NULL	0	NULL	proline betaine	AminoAcid		stimulate					E.coli	Organism	growth of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1420_1_30_s_335	10446288	Glycine betaine, choline and other urine constituents with dietary origins (e.g. proline betaine) stimulate growth of  E. coli, the primary causative agent of ascending urinary tract infections, in hypertonic media [  46].	transcription
60959	4	335658	7	NULL	NULL	0	NULL	E.coli	Organism		causative agent of					ascending urinary tract infections	medical finding				NULL	hypertonic media	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1420_1_30_s_335	10446288	Glycine betaine, choline and other urine constituents with dietary origins (e.g. proline betaine) stimulate growth of  E. coli, the primary causative agent of ascending urinary tract infections, in hypertonic media [  46].	transcription
56418	1	335659	5	NULL	NULL	0	NULL	OpuC			transports		efficiently			glycine betaine					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_560_s_10	0009925583	OpuC mediates the efficient transport not only of glycine betaine and choline- O-sulfate but also of carnitine, crotonobetaine, and gamma-butyrobetaine (R. Kappes and E. Bremer, Microbiology 144:83-90, 1998).	transcription
56419	2	335659	5	NULL	NULL	0	NULL	OpuC			transports		efficiently			choline- O-sulfate					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_560_s_10	0009925583	OpuC mediates the efficient transport not only of glycine betaine and choline- O-sulfate but also of carnitine, crotonobetaine, and gamma-butyrobetaine (R. Kappes and E. Bremer, Microbiology 144:83-90, 1998).	transcription
56420	3	335659	5	NULL	NULL	0	NULL	OpuC			transports		efficiently			carnitine					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_560_s_10	0009925583	OpuC mediates the efficient transport not only of glycine betaine and choline- O-sulfate but also of carnitine, crotonobetaine, and gamma-butyrobetaine (R. Kappes and E. Bremer, Microbiology 144:83-90, 1998).	transcription
56421	4	335659	5	NULL	NULL	0	NULL	OpuC			transports		efficiently			crotonobetaine					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_560_s_10	0009925583	OpuC mediates the efficient transport not only of glycine betaine and choline- O-sulfate but also of carnitine, crotonobetaine, and gamma-butyrobetaine (R. Kappes and E. Bremer, Microbiology 144:83-90, 1998).	transcription
56422	5	335659	5	NULL	NULL	0	NULL	OpuC			transports		efficiently			gamma-butyrobetaine					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_560_s_10	0009925583	OpuC mediates the efficient transport not only of glycine betaine and choline- O-sulfate but also of carnitine, crotonobetaine, and gamma-butyrobetaine (R. Kappes and E. Bremer, Microbiology 144:83-90, 1998).	transcription
60960	1	335659	7	NULL	NULL	0	NULL	OpuC	GP		mediates					glycine betaine	AminoAcid	efficient transport of			NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_560_s_10	0009925583	OpuC mediates the efficient transport not only of glycine betaine and choline- O-sulfate but also of carnitine, crotonobetaine, and gamma-butyrobetaine (R. Kappes and E. Bremer, Microbiology 144:83-90, 1998).	transcription
60961	2	335659	7	NULL	NULL	0	NULL	OpuC	GP		mediate					choline- O-sulfate	Chemical	efficient transport of			NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_560_s_10	0009925583	OpuC mediates the efficient transport not only of glycine betaine and choline- O-sulfate but also of carnitine, crotonobetaine, and gamma-butyrobetaine (R. Kappes and E. Bremer, Microbiology 144:83-90, 1998).	transcription
60962	3	335659	7	NULL	NULL	0	NULL	OpuC	GP		mediate					carnitine	Chemical	efficient transport of			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_560_s_10	0009925583	OpuC mediates the efficient transport not only of glycine betaine and choline- O-sulfate but also of carnitine, crotonobetaine, and gamma-butyrobetaine (R. Kappes and E. Bremer, Microbiology 144:83-90, 1998).	transcription
60963	4	335659	7	NULL	NULL	0	NULL	OpuC	GP		mediate					crotonobetaine	Chemical	efficient transport of			NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_560_s_10	0009925583	OpuC mediates the efficient transport not only of glycine betaine and choline- O-sulfate but also of carnitine, crotonobetaine, and gamma-butyrobetaine (R. Kappes and E. Bremer, Microbiology 144:83-90, 1998).	transcription
60964	5	335659	7	NULL	NULL	0	NULL	OpuC	GP		mediate					gamma-butyrobetaine	Chemical	efficient transport of			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_560_s_10	0009925583	OpuC mediates the efficient transport not only of glycine betaine and choline- O-sulfate but also of carnitine, crotonobetaine, and gamma-butyrobetaine (R. Kappes and E. Bremer, Microbiology 144:83-90, 1998).	transcription
60965	1	335660	7	NULL	NULL	0	NULL	glycine betaine gene	GP	neutrophilic;;Bacillus subtilis	is similar to					glycine betaine gene	GP	halotolerant;;Bacillus subtilis			NULL		0	NULL	NULL	NULL	gw70_femsmicrobiollett_235_2_393_s_14	15183890	Comparative analysis of this genome with that of the neutrophilic and halotolerant   Bacillus subtilis showed that there were no great differences in the genes of the glycine betaine and  choline ABC (ATP binding cassette) transport systems; however, a difference was found  in the glycine betaine secondary transporter genes [  18].	transcription
60966	2	335660	7	NULL	NULL	0	NULL	choline ABC gene	GP	neutrophilic;;Bacillus subtilis	is similar to					choline ABC gene	GP	halotolerant;;Bacillus subtilis			NULL		0	NULL	NULL	NULL	gw70_femsmicrobiollett_235_2_393_s_14	15183890	Comparative analysis of this genome with that of the neutrophilic and halotolerant   Bacillus subtilis showed that there were no great differences in the genes of the glycine betaine and  choline ABC (ATP binding cassette) transport systems; however, a difference was found  in the glycine betaine secondary transporter genes [  18].	transcription
60967	3	335660	7	NULL	NULL	0	NULL	glycine betaine secondary transporter genes	GP	neutrophilic;;Bacillus subtilis	is different from					glycine betaine secondary transporter genes	GP	halotolerant;;Bacillus subtilis			NULL		0	NULL	NULL	NULL	gw70_femsmicrobiollett_235_2_393_s_14	15183890	Comparative analysis of this genome with that of the neutrophilic and halotolerant   Bacillus subtilis showed that there were no great differences in the genes of the glycine betaine and  choline ABC (ATP binding cassette) transport systems; however, a difference was found  in the glycine betaine secondary transporter genes [  18].	transcription
60968	4	335660	7	NULL	NULL	0	NULL	ABC	GP		is					ATP binding cassette	GP				NULL		0	NULL	NULL	NULL	gw70_femsmicrobiollett_235_2_393_s_14	15183890	Comparative analysis of this genome with that of the neutrophilic and halotolerant   Bacillus subtilis showed that there were no great differences in the genes of the glycine betaine and  choline ABC (ATP binding cassette) transport systems; however, a difference was found  in the glycine betaine secondary transporter genes [  18].	transcription
56423	1	335661	5	NULL	NULL	0	NULL	ProX protein		E. coli	bind		high affinity			proline betaine					NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_50_0_101_s_244	8905077	The  E.  coli ProX protein binds both proline betaine and glycine betaine with high affinity [e.g.   Kd 5.2  M for proline betaine and 1.4  M for glycine betaine ( 57)], yet ProX does not bind the low affinity ProU substrates proline and choline ( 26).	transcription
56424	2	335661	5	NULL	NULL	0	NULL	ProX protein		E. coli	bind		high affinity			glycine betaine					NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_50_0_101_s_244	8905077	The  E.  coli ProX protein binds both proline betaine and glycine betaine with high affinity [e.g.   Kd 5.2  M for proline betaine and 1.4  M for glycine betaine ( 57)], yet ProX does not bind the low affinity ProU substrates proline and choline ( 26).	transcription
56425	3	335661	5	NULL	NULL	0	NULL	proline			substrate of					ProU					NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_50_0_101_s_244	8905077	The  E.  coli ProX protein binds both proline betaine and glycine betaine with high affinity [e.g.   Kd 5.2  M for proline betaine and 1.4  M for glycine betaine ( 57)], yet ProX does not bind the low affinity ProU substrates proline and choline ( 26).	transcription
56427	4	335661	5	NULL	NULL	0	NULL	choline			substrate of					ProU 					NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_50_0_101_s_244	8905077	The  E.  coli ProX protein binds both proline betaine and glycine betaine with high affinity [e.g.   Kd 5.2  M for proline betaine and 1.4  M for glycine betaine ( 57)], yet ProX does not bind the low affinity ProU substrates proline and choline ( 26).	transcription
56428	5	335661	5	NULL	NULL	0	NULL	ProX protein		E. coli	does not bind					proline					NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_50_0_101_s_244	8905077	The  E.  coli ProX protein binds both proline betaine and glycine betaine with high affinity [e.g.   Kd 5.2  M for proline betaine and 1.4  M for glycine betaine ( 57)], yet ProX does not bind the low affinity ProU substrates proline and choline ( 26).	transcription
56429	6	335661	5	NULL	NULL	0	NULL	ProX protein		E. coli	does not bind					choline					NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_50_0_101_s_244	8905077	The  E.  coli ProX protein binds both proline betaine and glycine betaine with high affinity [e.g.   Kd 5.2  M for proline betaine and 1.4  M for glycine betaine ( 57)], yet ProX does not bind the low affinity ProU substrates proline and choline ( 26).	transcription
60969	1	335661	7	NULL	NULL	0	NULL	ProX protein	GP	E.coli	bind		high affinity			proline betaine	AminoAcid				NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_50_0_101_s_244	8905077	The  E.  coli ProX protein binds both proline betaine and glycine betaine with high affinity [e.g.   Kd 5.2  M for proline betaine and 1.4  M for glycine betaine ( 57)], yet ProX does not bind the low affinity ProU substrates proline and choline ( 26).	transcription
60970	2	335661	7	NULL	NULL	0	NULL	ProX protein	GP	E.coli	bind		high affinity			glycine betaine	AminoAcid				NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_50_0_101_s_244	8905077	The  E.  coli ProX protein binds both proline betaine and glycine betaine with high affinity [e.g.   Kd 5.2  M for proline betaine and 1.4  M for glycine betaine ( 57)], yet ProX does not bind the low affinity ProU substrates proline and choline ( 26).	transcription
60971	3	335661	7	NULL	NULL	0	NULL	ProX	GP		does not bind					proline	AminoAcid				NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_50_0_101_s_244	8905077	The  E.  coli ProX protein binds both proline betaine and glycine betaine with high affinity [e.g.   Kd 5.2  M for proline betaine and 1.4  M for glycine betaine ( 57)], yet ProX does not bind the low affinity ProU substrates proline and choline ( 26).	transcription
60972	4	335661	7	NULL	NULL	0	NULL	ProX	GP		does not bind					choline	Chemical				NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_50_0_101_s_244	8905077	The  E.  coli ProX protein binds both proline betaine and glycine betaine with high affinity [e.g.   Kd 5.2  M for proline betaine and 1.4  M for glycine betaine ( 57)], yet ProX does not bind the low affinity ProU substrates proline and choline ( 26).	transcription
60973	5	335661	7	NULL	NULL	0	NULL	proline	AminoAcid		is a type of					ProU substrate	GP	low affinity			NULL		NULL	NULL	NULL	NULL	gw70_annurevmicrobiol_50_0_101_s_244	8905077	The  E.  coli ProX protein binds both proline betaine and glycine betaine with high affinity [e.g.   Kd 5.2  M for proline betaine and 1.4  M for glycine betaine ( 57)], yet ProX does not bind the low affinity ProU substrates proline and choline ( 26).	transcription
60974	6	335661	7	NULL	NULL	0	NULL	choline	Chemical		is a type of					ProU substrate	GP	low affinity			NULL		0	NULL	NULL	NULL	gw70_annurevmicrobiol_50_0_101_s_244	8905077	The  E.  coli ProX protein binds both proline betaine and glycine betaine with high affinity [e.g.   Kd 5.2  M for proline betaine and 1.4  M for glycine betaine ( 57)], yet ProX does not bind the low affinity ProU substrates proline and choline ( 26).	transcription
60975	1	335662	7	NULL	NULL	0	NULL	RpoS	GP	expression of	regulate					osmY	GP				NULL		NULL	NULL	NULL	NULL	gw70_applenvironmicrob_69_3_1759_s_273	12620868	Besides the expression of RpoS-regulated  osmY, the expression of the  betIBA operon for the synthesis of the compatible solute glycine betaine from choline, of the  proVWX operon for the uptake of proline and glycine betaine, and of the  otsAB operon for the synthesis of the compatible solute trehalose was increased after adaptation to acetate or propionate.	transcription
60976	2	335662	7	NULL	NULL	0	NULL	glycine betaine	AminoAcid		synthesized from					choline	Chemical				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_3_1759_s_273	12620868	Besides the expression of RpoS-regulated  osmY, the expression of the  betIBA operon for the synthesis of the compatible solute glycine betaine from choline, of the  proVWX operon for the uptake of proline and glycine betaine, and of the  otsAB operon for the synthesis of the compatible solute trehalose was increased after adaptation to acetate or propionate.	transcription
60977	3	335662	7	NULL	NULL	0	NULL	betIBA operon	GP	expression of	is required for					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_3_1759_s_273	12620868	Besides the expression of RpoS-regulated  osmY, the expression of the  betIBA operon for the synthesis of the compatible solute glycine betaine from choline, of the  proVWX operon for the uptake of proline and glycine betaine, and of the  otsAB operon for the synthesis of the compatible solute trehalose was increased after adaptation to acetate or propionate.	transcription
60978	4	335662	7	NULL	NULL	0	NULL	proVWX operon	GP	expression of	is required for					proline	AminoAcid	uptake of			NULL		NULL	NULL	NULL	NULL	gw70_applenvironmicrob_69_3_1759_s_273	12620868	Besides the expression of RpoS-regulated  osmY, the expression of the  betIBA operon for the synthesis of the compatible solute glycine betaine from choline, of the  proVWX operon for the uptake of proline and glycine betaine, and of the  otsAB operon for the synthesis of the compatible solute trehalose was increased after adaptation to acetate or propionate.	transcription
60979	5	335662	7	NULL	NULL	0	NULL	proVWX operon	GP	expression of	is required for					glycine betaine	AminoAcid	uptake of			NULL		NULL	NULL	NULL	NULL	gw70_applenvironmicrob_69_3_1759_s_273	12620868	Besides the expression of RpoS-regulated  osmY, the expression of the  betIBA operon for the synthesis of the compatible solute glycine betaine from choline, of the  proVWX operon for the uptake of proline and glycine betaine, and of the  otsAB operon for the synthesis of the compatible solute trehalose was increased after adaptation to acetate or propionate.	transcription
60980	6	335662	7	NULL	NULL	0	NULL	otsAB operon	GP	expression of	is required for					trehalose	Chemical	synthesis of;;compatible solute			NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_3_1759_s_273	12620868	Besides the expression of RpoS-regulated  osmY, the expression of the  betIBA operon for the synthesis of the compatible solute glycine betaine from choline, of the  proVWX operon for the uptake of proline and glycine betaine, and of the  otsAB operon for the synthesis of the compatible solute trehalose was increased after adaptation to acetate or propionate.	transcription
60981	7	335662	7	NULL	NULL	0	NULL	acetate	Chemical		increase					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_3_1759_s_273	12620868	Besides the expression of RpoS-regulated  osmY, the expression of the  betIBA operon for the synthesis of the compatible solute glycine betaine from choline, of the  proVWX operon for the uptake of proline and glycine betaine, and of the  otsAB operon for the synthesis of the compatible solute trehalose was increased after adaptation to acetate or propionate.	transcription
60982	8	335662	7	NULL	NULL	0	NULL	propionate	Chemical		increase					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_3_1759_s_273	12620868	Besides the expression of RpoS-regulated  osmY, the expression of the  betIBA operon for the synthesis of the compatible solute glycine betaine from choline, of the  proVWX operon for the uptake of proline and glycine betaine, and of the  otsAB operon for the synthesis of the compatible solute trehalose was increased after adaptation to acetate or propionate.	transcription
60983	9	335662	7	NULL	NULL	0	NULL	acetate	Chemical		increase					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_3_1759_s_273	12620868	Besides the expression of RpoS-regulated  osmY, the expression of the  betIBA operon for the synthesis of the compatible solute glycine betaine from choline, of the  proVWX operon for the uptake of proline and glycine betaine, and of the  otsAB operon for the synthesis of the compatible solute trehalose was increased after adaptation to acetate or propionate.	transcription
60984	10	335662	7	NULL	NULL	0	NULL	propionate	Chemical		increase					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_3_1759_s_273	12620868	Besides the expression of RpoS-regulated  osmY, the expression of the  betIBA operon for the synthesis of the compatible solute glycine betaine from choline, of the  proVWX operon for the uptake of proline and glycine betaine, and of the  otsAB operon for the synthesis of the compatible solute trehalose was increased after adaptation to acetate or propionate.	transcription
60985	11	335662	7	NULL	NULL	0	NULL	acetate	Chemical		increase					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_3_1759_s_273	12620868	Besides the expression of RpoS-regulated  osmY, the expression of the  betIBA operon for the synthesis of the compatible solute glycine betaine from choline, of the  proVWX operon for the uptake of proline and glycine betaine, and of the  otsAB operon for the synthesis of the compatible solute trehalose was increased after adaptation to acetate or propionate.	transcription
60986	12	335662	7	NULL	NULL	0	NULL	propionate	Chemical		increase					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_3_1759_s_273	12620868	Besides the expression of RpoS-regulated  osmY, the expression of the  betIBA operon for the synthesis of the compatible solute glycine betaine from choline, of the  proVWX operon for the uptake of proline and glycine betaine, and of the  otsAB operon for the synthesis of the compatible solute trehalose was increased after adaptation to acetate or propionate.	transcription
60987	13	335662	7	NULL	NULL	0	NULL	acetate	Chemical		increase					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_applenvironmicrob_69_3_1759_s_273	12620868	Besides the expression of RpoS-regulated  osmY, the expression of the  betIBA operon for the synthesis of the compatible solute glycine betaine from choline, of the  proVWX operon for the uptake of proline and glycine betaine, and of the  otsAB operon for the synthesis of the compatible solute trehalose was increased after adaptation to acetate or propionate.	transcription
60988	14	335662	7	NULL	NULL	0	NULL	propionate	Chemical		increase					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_3_1759_s_273	12620868	Besides the expression of RpoS-regulated  osmY, the expression of the  betIBA operon for the synthesis of the compatible solute glycine betaine from choline, of the  proVWX operon for the uptake of proline and glycine betaine, and of the  otsAB operon for the synthesis of the compatible solute trehalose was increased after adaptation to acetate or propionate.	transcription
60989	15	335662	7	NULL	NULL	0	NULL	acetate	Chemical		increase					statement 6	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_3_1759_s_273	12620868	Besides the expression of RpoS-regulated  osmY, the expression of the  betIBA operon for the synthesis of the compatible solute glycine betaine from choline, of the  proVWX operon for the uptake of proline and glycine betaine, and of the  otsAB operon for the synthesis of the compatible solute trehalose was increased after adaptation to acetate or propionate.	transcription
60990	16	335662	7	NULL	NULL	0	NULL	propionate	Chemical		increase					statement 6	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_69_3_1759_s_273	12620868	Besides the expression of RpoS-regulated  osmY, the expression of the  betIBA operon for the synthesis of the compatible solute glycine betaine from choline, of the  proVWX operon for the uptake of proline and glycine betaine, and of the  otsAB operon for the synthesis of the compatible solute trehalose was increased after adaptation to acetate or propionate.	transcription
56431	1	335664	5	NULL	NULL	0	NULL	Hut system			is transport system for					betaines					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_10_5916_s_27	15466533	Two transport systems for betaines have been fully characterized: the Hut system, an ATP-binding cassette histidine transporter also involved in low-affinity glycine betaine transport ( ), and the BetS system, a betaine choline carnitine transporter (BCCT) required for early osmotic adjustment ( ).	transcription
56432	2	335664	5	NULL	NULL	0	NULL	BetS system			is transport system for					betaines					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_10_5916_s_27	15466533	Two transport systems for betaines have been fully characterized: the Hut system, an ATP-binding cassette histidine transporter also involved in low-affinity glycine betaine transport ( ), and the BetS system, a betaine choline carnitine transporter (BCCT) required for early osmotic adjustment ( ).	transcription
56433	3	335664	5	NULL	NULL	0	NULL	Hut system			is a type of					ATP-binding cassette histidine transporter					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_10_5916_s_27	15466533	Two transport systems for betaines have been fully characterized: the Hut system, an ATP-binding cassette histidine transporter also involved in low-affinity glycine betaine transport ( ), and the BetS system, a betaine choline carnitine transporter (BCCT) required for early osmotic adjustment ( ).	transcription
56434	4	335664	5	NULL	NULL	0	NULL	Hut system			is involved in					glycine betaine		transport of;;low-affinity			NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_10_5916_s_27	15466533	Two transport systems for betaines have been fully characterized: the Hut system, an ATP-binding cassette histidine transporter also involved in low-affinity glycine betaine transport ( ), and the BetS system, a betaine choline carnitine transporter (BCCT) required for early osmotic adjustment ( ).	transcription
56435	5	335664	5	NULL	NULL	0	NULL	BetS system			is a type of					betaine choline carnitine transporter					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_10_5916_s_27	15466533	Two transport systems for betaines have been fully characterized: the Hut system, an ATP-binding cassette histidine transporter also involved in low-affinity glycine betaine transport ( ), and the BetS system, a betaine choline carnitine transporter (BCCT) required for early osmotic adjustment ( ).	transcription
56436	6	335664	5	NULL	NULL	0	NULL	BCC			is
\n					betaine choline carnitine transporter					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_10_5916_s_27	15466533	Two transport systems for betaines have been fully characterized: the Hut system, an ATP-binding cassette histidine transporter also involved in low-affinity glycine betaine transport ( ), and the BetS system, a betaine choline carnitine transporter (BCCT) required for early osmotic adjustment ( ).	transcription
56437	7	335664	5	NULL	NULL	0	NULL	BetS system			is required for					osmotic adjustment 		early			NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_10_5916_s_27	15466533	Two transport systems for betaines have been fully characterized: the Hut system, an ATP-binding cassette histidine transporter also involved in low-affinity glycine betaine transport ( ), and the BetS system, a betaine choline carnitine transporter (BCCT) required for early osmotic adjustment ( ).	transcription
60991	1	335664	7	NULL	NULL	0	NULL	Hut system	GP		is a type of					ATP-binding cassette histidine transporter	GP				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_10_5916_s_27	15466533	Two transport systems for betaines have been fully characterized: the Hut system, an ATP-binding cassette histidine transporter also involved in low-affinity glycine betaine transport ( ), and the BetS system, a betaine choline carnitine transporter (BCCT) required for early osmotic adjustment ( ).	transcription
60992	2	335664	7	NULL	NULL	0	NULL	statement 1	Process		is involved in					glycine betaine	AminoAcid	low-affinity transport of			NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_10_5916_s_27	15466533	Two transport systems for betaines have been fully characterized: the Hut system, an ATP-binding cassette histidine transporter also involved in low-affinity glycine betaine transport ( ), and the BetS system, a betaine choline carnitine transporter (BCCT) required for early osmotic adjustment ( ).	transcription
60993	3	335664	7	NULL	NULL	0	NULL	BetS system	GP		is a type of					BCCT	GP				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_10_5916_s_27	15466533	Two transport systems for betaines have been fully characterized: the Hut system, an ATP-binding cassette histidine transporter also involved in low-affinity glycine betaine transport ( ), and the BetS system, a betaine choline carnitine transporter (BCCT) required for early osmotic adjustment ( ).	transcription
60994	4	335664	7	NULL	NULL	0	NULL	statement 3	Process		is required for					early osmotic adjustment	Process				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_10_5916_s_27	15466533	Two transport systems for betaines have been fully characterized: the Hut system, an ATP-binding cassette histidine transporter also involved in low-affinity glycine betaine transport ( ), and the BetS system, a betaine choline carnitine transporter (BCCT) required for early osmotic adjustment ( ).	transcription
60995	5	335664	7	NULL	NULL	0	NULL	BCCT	GP		is 					betaine choline carnitine transporter	GP				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_70_10_5916_s_27	15466533	Two transport systems for betaines have been fully characterized: the Hut system, an ATP-binding cassette histidine transporter also involved in low-affinity glycine betaine transport ( ), and the BetS system, a betaine choline carnitine transporter (BCCT) required for early osmotic adjustment ( ).	transcription
56438	1	335665	5	NULL	NULL	0	NULL	ABC transporters			mediates					choline		uptake of			NULL	Bacillus subtilis	0	NULL	NULL	NULL	gw60_femsmicrobiolrev_26_1_49_s_918	12007642	R.M. Kappes, B. Kempf, S. Kneip, J. Boch, J. Gade, J. Meier-Wagner and E. Bremer, Two evolutionary closely related ABC transporters mediate the uptake of choline for synthesis of the osmoprotectant glycine betaine in  Bacillus subtilis.	transcription
56439	2	335665	5	NULL	NULL	0	NULL	statement 1			is required for					glycine betaine		synthesis of			NULL	Bacillus subtilis	0	NULL	NULL	NULL	gw60_femsmicrobiolrev_26_1_49_s_918	12007642	R.M. Kappes, B. Kempf, S. Kneip, J. Boch, J. Gade, J. Meier-Wagner and E. Bremer, Two evolutionary closely related ABC transporters mediate the uptake of choline for synthesis of the osmoprotectant glycine betaine in  Bacillus subtilis.	transcription
56440	3	335665	5	NULL	NULL	0	NULL	glycine betaine			is a type of					osmoprotectant					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiolrev_26_1_49_s_918	12007642	R.M. Kappes, B. Kempf, S. Kneip, J. Boch, J. Gade, J. Meier-Wagner and E. Bremer, Two evolutionary closely related ABC transporters mediate the uptake of choline for synthesis of the osmoprotectant glycine betaine in  Bacillus subtilis.	transcription
60996	1	335665	7	NULL	NULL	0	NULL	ABC transporters	GP		mediate					choline	Chemical	uptake of			NULL		0	NULL	NULL	NULL	gw60_femsmicrobiolrev_26_1_49_s_918	12007642	R.M. Kappes, B. Kempf, S. Kneip, J. Boch, J. Gade, J. Meier-Wagner and E. Bremer, Two evolutionary closely related ABC transporters mediate the uptake of choline for synthesis of the osmoprotectant glycine betaine in  Bacillus subtilis.	transcription
60997	2	335665	7	NULL	NULL	0	NULL	statement 1	Process		is required for 					glycine betaine	AminoAcid	synthesis of			NULL	Bacillus subtilis	NULL	NULL	NULL	NULL	gw60_femsmicrobiolrev_26_1_49_s_918	12007642	R.M. Kappes, B. Kempf, S. Kneip, J. Boch, J. Gade, J. Meier-Wagner and E. Bremer, Two evolutionary closely related ABC transporters mediate the uptake of choline for synthesis of the osmoprotectant glycine betaine in  Bacillus subtilis.	transcription
60998	3	335665	7	NULL	NULL	0	NULL	glycine betaine	AminoAcid		is a type of					osmoprotectant	Process				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiolrev_26_1_49_s_918	12007642	R.M. Kappes, B. Kempf, S. Kneip, J. Boch, J. Gade, J. Meier-Wagner and E. Bremer, Two evolutionary closely related ABC transporters mediate the uptake of choline for synthesis of the osmoprotectant glycine betaine in  Bacillus subtilis.	transcription
56441	1	335667	5	NULL	NULL	0	NULL	mAChRs			is present in					glycinergic amacrine cells					NULL	rabbit retina	0	NULL	NULL	NULL	gw60_jneurosci_20_22_8417_s_208	11069949	For instance, in rabbit retina, mAChRs on glycinergic amacrine cells stimulate the release of glycine, which then inhibits release of ACh from cholinergic amacrine cells (Cunningham et al., 1983  ; Neal and Cunningham, 1995  ; Linn, 1998  ).	transcription
56442	2	335667	5	NULL	NULL	0	NULL	statement 1			stimulates					glycine		release of			NULL	rabbit retina	0	NULL	NULL	NULL	gw60_jneurosci_20_22_8417_s_208	11069949	For instance, in rabbit retina, mAChRs on glycinergic amacrine cells stimulate the release of glycine, which then inhibits release of ACh from cholinergic amacrine cells (Cunningham et al., 1983  ; Neal and Cunningham, 1995  ; Linn, 1998  ).	transcription
56443	3	335667	5	NULL	NULL	0	NULL	ACh			is released from					cholinergic amacrine cells					NULL	rabbit retina	NULL	NULL	NULL	NULL	gw60_jneurosci_20_22_8417_s_208	11069949	For instance, in rabbit retina, mAChRs on glycinergic amacrine cells stimulate the release of glycine, which then inhibits release of ACh from cholinergic amacrine cells (Cunningham et al., 1983  ; Neal and Cunningham, 1995  ; Linn, 1998  ).	transcription
56444	4	335667	5	NULL	NULL	0	NULL	statement 3			inhibits					statement 2					NULL		0	NULL	NULL	NULL	gw60_jneurosci_20_22_8417_s_208	11069949	For instance, in rabbit retina, mAChRs on glycinergic amacrine cells stimulate the release of glycine, which then inhibits release of ACh from cholinergic amacrine cells (Cunningham et al., 1983  ; Neal and Cunningham, 1995  ; Linn, 1998  ).	transcription
60999	1	335667	7	NULL	NULL	0	NULL	mAChRs	GP	rabbit retina	stimulate					glycine	AminoAcid	release of			NULL	glycinergic amacrine cells	0	NULL	NULL	NULL	gw60_jneurosci_20_22_8417_s_208	11069949	For instance, in rabbit retina, mAChRs on glycinergic amacrine cells stimulate the release of glycine, which then inhibits release of ACh from cholinergic amacrine cells (Cunningham et al., 1983  ; Neal and Cunningham, 1995  ; Linn, 1998  ).	transcription
61000	2	335667	7	NULL	NULL	0	NULL	glycine	AminoAcid		inhibit					ACh	GP	release of			NULL	cholinergic amacrine cells 	0	NULL	NULL	NULL	gw60_jneurosci_20_22_8417_s_208	11069949	For instance, in rabbit retina, mAChRs on glycinergic amacrine cells stimulate the release of glycine, which then inhibits release of ACh from cholinergic amacrine cells (Cunningham et al., 1983  ; Neal and Cunningham, 1995  ; Linn, 1998  ).	transcription
56445	1	335668	5	NULL	NULL	0	NULL	opuCA			encodes					glycine/betaine/carnitine/choline ABC transporter					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_8_5197_s_29	16885265	To do this, transcript levels were determined for  opuCA, which encodes a glycine/betaine/carnitine/choline ABC transporter ( ,  ,  ,  ,  ), and for  clpC, which encodes endopeptidase Clp ATP-binding chain C, a stress response protein that contributes to  L. monocytogenes phagosomal escape ( ,  ,  ), in the  L. monocytogenes wild-type, delta sigB, delta rsbT, and delta rsbV strains under different stress conditions.	transcription
56446	2	335668	5	NULL	NULL	0	NULL	clpC			encodes					endopeptidase Clp			ATP-binding chain C		NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_8_5197_s_29	16885265	To do this, transcript levels were determined for  opuCA, which encodes a glycine/betaine/carnitine/choline ABC transporter ( ,  ,  ,  ,  ), and for  clpC, which encodes endopeptidase Clp ATP-binding chain C, a stress response protein that contributes to  L. monocytogenes phagosomal escape ( ,  ,  ), in the  L. monocytogenes wild-type, delta sigB, delta rsbT, and delta rsbV strains under different stress conditions.	transcription
56447	3	335668	5	NULL	NULL	0	NULL	endopeptidase Clp			is a type of			ATP-binding chain C		stress response protein					NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_8_5197_s_29	16885265	To do this, transcript levels were determined for  opuCA, which encodes a glycine/betaine/carnitine/choline ABC transporter ( ,  ,  ,  ,  ), and for  clpC, which encodes endopeptidase Clp ATP-binding chain C, a stress response protein that contributes to  L. monocytogenes phagosomal escape ( ,  ,  ), in the  L. monocytogenes wild-type, delta sigB, delta rsbT, and delta rsbV strains under different stress conditions.	transcription
56448	4	335668	5	NULL	NULL	0	NULL	endopeptidase Clp			contributes to			ATP-binding chain C		L. monocytogenes		phagosomal escape of			NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_8_5197_s_29	16885265	To do this, transcript levels were determined for  opuCA, which encodes a glycine/betaine/carnitine/choline ABC transporter ( ,  ,  ,  ,  ), and for  clpC, which encodes endopeptidase Clp ATP-binding chain C, a stress response protein that contributes to  L. monocytogenes phagosomal escape ( ,  ,  ), in the  L. monocytogenes wild-type, delta sigB, delta rsbT, and delta rsbV strains under different stress conditions.	transcription
61001	1	335668	7	NULL	NULL	0	NULL	opuCA	GP		encode					glycine ABC transporter	GP				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_8_5197_s_29	16885265	To do this, transcript levels were determined for  opuCA, which encodes a glycine/betaine/carnitine/choline ABC transporter ( ,  ,  ,  ,  ), and for  clpC, which encodes endopeptidase Clp ATP-binding chain C, a stress response protein that contributes to  L. monocytogenes phagosomal escape ( ,  ,  ), in the  L. monocytogenes wild-type, delta sigB, delta rsbT, and delta rsbV strains under different stress conditions.	transcription
61002	2	335668	7	NULL	NULL	0	NULL	opuCA	GP		encode					betaine ABC transporter	GP				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_8_5197_s_29	16885265	To do this, transcript levels were determined for  opuCA, which encodes a glycine/betaine/carnitine/choline ABC transporter ( ,  ,  ,  ,  ), and for  clpC, which encodes endopeptidase Clp ATP-binding chain C, a stress response protein that contributes to  L. monocytogenes phagosomal escape ( ,  ,  ), in the  L. monocytogenes wild-type, delta sigB, delta rsbT, and delta rsbV strains under different stress conditions.	transcription
61003	3	335668	7	NULL	NULL	0	NULL	opuCA	GP		encode					carnitine ABC transporter	GP				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_8_5197_s_29	16885265	To do this, transcript levels were determined for  opuCA, which encodes a glycine/betaine/carnitine/choline ABC transporter ( ,  ,  ,  ,  ), and for  clpC, which encodes endopeptidase Clp ATP-binding chain C, a stress response protein that contributes to  L. monocytogenes phagosomal escape ( ,  ,  ), in the  L. monocytogenes wild-type, delta sigB, delta rsbT, and delta rsbV strains under different stress conditions.	transcription
61004	4	335668	7	NULL	NULL	0	NULL	opuCA	GP		encode					choline ABC transporter	GP				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_8_5197_s_29	16885265	To do this, transcript levels were determined for  opuCA, which encodes a glycine/betaine/carnitine/choline ABC transporter ( ,  ,  ,  ,  ), and for  clpC, which encodes endopeptidase Clp ATP-binding chain C, a stress response protein that contributes to  L. monocytogenes phagosomal escape ( ,  ,  ), in the  L. monocytogenes wild-type, delta sigB, delta rsbT, and delta rsbV strains under different stress conditions.	transcription
61005	5	335668	7	NULL	NULL	0	NULL	clpC	GP		encode					endopeptidase Clp ATP-binding chain C	GP				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_8_5197_s_29	16885265	To do this, transcript levels were determined for  opuCA, which encodes a glycine/betaine/carnitine/choline ABC transporter ( ,  ,  ,  ,  ), and for  clpC, which encodes endopeptidase Clp ATP-binding chain C, a stress response protein that contributes to  L. monocytogenes phagosomal escape ( ,  ,  ), in the  L. monocytogenes wild-type, delta sigB, delta rsbT, and delta rsbV strains under different stress conditions.	transcription
61006	6	335668	7	NULL	NULL	0	NULL	endopeptidase Clp ATP-binding chain C	GP		contributes to					phagosomal escape	Process				NULL	wild-type L. monocytogenes	0	NULL	NULL	NULL	gw70_applenvironmicrob_72_8_5197_s_29	16885265	To do this, transcript levels were determined for  opuCA, which encodes a glycine/betaine/carnitine/choline ABC transporter ( ,  ,  ,  ,  ), and for  clpC, which encodes endopeptidase Clp ATP-binding chain C, a stress response protein that contributes to  L. monocytogenes phagosomal escape ( ,  ,  ), in the  L. monocytogenes wild-type, delta sigB, delta rsbT, and delta rsbV strains under different stress conditions.	transcription
61007	7	335668	7	NULL	NULL	0	NULL	endopeptidase Clp ATP-binding chain C	GP		contributes to					phagosomal escape	Process				NULL	delta sigB L. monocytogenes	0	NULL	NULL	NULL	gw70_applenvironmicrob_72_8_5197_s_29	16885265	To do this, transcript levels were determined for  opuCA, which encodes a glycine/betaine/carnitine/choline ABC transporter ( ,  ,  ,  ,  ), and for  clpC, which encodes endopeptidase Clp ATP-binding chain C, a stress response protein that contributes to  L. monocytogenes phagosomal escape ( ,  ,  ), in the  L. monocytogenes wild-type, delta sigB, delta rsbT, and delta rsbV strains under different stress conditions.	transcription
61008	8	335668	7	NULL	NULL	0	NULL	endopeptidase Clp ATP-binding chain C	GP		contributes to					phagosomal escape	Process				NULL	delta rsbT L. monocytogenes	0	NULL	NULL	NULL	gw70_applenvironmicrob_72_8_5197_s_29	16885265	To do this, transcript levels were determined for  opuCA, which encodes a glycine/betaine/carnitine/choline ABC transporter ( ,  ,  ,  ,  ), and for  clpC, which encodes endopeptidase Clp ATP-binding chain C, a stress response protein that contributes to  L. monocytogenes phagosomal escape ( ,  ,  ), in the  L. monocytogenes wild-type, delta sigB, delta rsbT, and delta rsbV strains under different stress conditions.	transcription
61009	9	335668	7	NULL	NULL	0	NULL	endopeptidase Clp ATP-binding chain C	GP		contributes to					phagosomal escape	Process				NULL	delta rsbV L. monocytogenes	0	NULL	NULL	NULL	gw70_applenvironmicrob_72_8_5197_s_29	16885265	To do this, transcript levels were determined for  opuCA, which encodes a glycine/betaine/carnitine/choline ABC transporter ( ,  ,  ,  ,  ), and for  clpC, which encodes endopeptidase Clp ATP-binding chain C, a stress response protein that contributes to  L. monocytogenes phagosomal escape ( ,  ,  ), in the  L. monocytogenes wild-type, delta sigB, delta rsbT, and delta rsbV strains under different stress conditions.	transcription
61010	10	335668	7	NULL	NULL	0	NULL	endopeptidase Clp ATP-binding chain C	GP		is a type of					stress response protein	GP				NULL		0	NULL	NULL	NULL	gw70_applenvironmicrob_72_8_5197_s_29	16885265	To do this, transcript levels were determined for  opuCA, which encodes a glycine/betaine/carnitine/choline ABC transporter ( ,  ,  ,  ,  ), and for  clpC, which encodes endopeptidase Clp ATP-binding chain C, a stress response protein that contributes to  L. monocytogenes phagosomal escape ( ,  ,  ), in the  L. monocytogenes wild-type, delta sigB, delta rsbT, and delta rsbV strains under different stress conditions.	transcription
56450	1	335670	5	NULL	NULL	0	NULL	rCBF response			abolished by					scopolamine					NULL		0	NULL	NULL	NULL	gw60_brainres_832_1_118_s_98	10375657	-Cycloserine significantly recovered the rCBF response abolished by scopolamine in our previous study without affecting neuronal activity, suggesting that the activation of NMDA receptors through the glycine site by  -cycloserine could reverse the dysfunction in the coupling between neuronal activation and the rCBF response that is associated with a cholinergic blockade [ 43].	transcription
56451	2	335670	5	NULL	NULL	0	NULL	statement 1			does not affect					neuronal activity					NULL		0	NULL	NULL	NULL	gw60_brainres_832_1_118_s_98	10375657	-Cycloserine significantly recovered the rCBF response abolished by scopolamine in our previous study without affecting neuronal activity, suggesting that the activation of NMDA receptors through the glycine site by  -cycloserine could reverse the dysfunction in the coupling between neuronal activation and the rCBF response that is associated with a cholinergic blockade [ 43].	transcription
56452	3	335670	5	NULL	NULL	0	NULL	Cycloserine			recover		significantly			statement 1					NULL		0	NULL	NULL	NULL	gw60_brainres_832_1_118_s_98	10375657	-Cycloserine significantly recovered the rCBF response abolished by scopolamine in our previous study without affecting neuronal activity, suggesting that the activation of NMDA receptors through the glycine site by  -cycloserine could reverse the dysfunction in the coupling between neuronal activation and the rCBF response that is associated with a cholinergic blockade [ 43].	transcription
56453	4	335670	5	NULL	NULL	0	NULL	cycloserine			activates					NMDA receptor					NULL		0	NULL	NULL	NULL	gw60_brainres_832_1_118_s_98	10375657	-Cycloserine significantly recovered the rCBF response abolished by scopolamine in our previous study without affecting neuronal activity, suggesting that the activation of NMDA receptors through the glycine site by  -cycloserine could reverse the dysfunction in the coupling between neuronal activation and the rCBF response that is associated with a cholinergic blockade [ 43].	transcription
56454	5	335670	5	NULL	NULL	0	NULL	statement 4			through					glycine site					NULL		0	NULL	NULL	NULL	gw60_brainres_832_1_118_s_98	10375657	-Cycloserine significantly recovered the rCBF response abolished by scopolamine in our previous study without affecting neuronal activity, suggesting that the activation of NMDA receptors through the glycine site by  -cycloserine could reverse the dysfunction in the coupling between neuronal activation and the rCBF response that is associated with a cholinergic blockade [ 43].	transcription
56455	6	335670	5	NULL	NULL	0	NULL	rCBF response			is associated with					cholinergic blockade					NULL		0	NULL	NULL	NULL	gw60_brainres_832_1_118_s_98	10375657	-Cycloserine significantly recovered the rCBF response abolished by scopolamine in our previous study without affecting neuronal activity, suggesting that the activation of NMDA receptors through the glycine site by  -cycloserine could reverse the dysfunction in the coupling between neuronal activation and the rCBF response that is associated with a cholinergic blockade [ 43].	transcription
56456	7	335670	5	NULL	NULL	0	NULL	neuronal activation			is coupled to					rCBF response					NULL		0	NULL	NULL	NULL	gw60_brainres_832_1_118_s_98	10375657	-Cycloserine significantly recovered the rCBF response abolished by scopolamine in our previous study without affecting neuronal activity, suggesting that the activation of NMDA receptors through the glycine site by  -cycloserine could reverse the dysfunction in the coupling between neuronal activation and the rCBF response that is associated with a cholinergic blockade [ 43].	transcription
56457	8	335670	5	NULL	NULL	0	NULL	statement 4			reverse					statement 7		dysfunction of			NULL		0	NULL	NULL	NULL	gw60_brainres_832_1_118_s_98	10375657	-Cycloserine significantly recovered the rCBF response abolished by scopolamine in our previous study without affecting neuronal activity, suggesting that the activation of NMDA receptors through the glycine site by  -cycloserine could reverse the dysfunction in the coupling between neuronal activation and the rCBF response that is associated with a cholinergic blockade [ 43].	transcription
61038	1	335670	7	NULL	NULL	0	NULL	scopolamine	Chemical		abolish					 rCBF response	Process				NULL		0	NULL	NULL	NULL	gw60_brainres_832_1_118_s_98	10375657	-Cycloserine significantly recovered the rCBF response abolished by scopolamine in our previous study without affecting neuronal activity, suggesting that the activation of NMDA receptors through the glycine site by  -cycloserine could reverse the dysfunction in the coupling between neuronal activation and the rCBF response that is associated with a cholinergic blockade [ 43].	transcription
61039	2	335670	7	NULL	NULL	0	NULL	Cycloserine 	Chemical		recovers		significantly			statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_brainres_832_1_118_s_98	10375657	-Cycloserine significantly recovered the rCBF response abolished by scopolamine in our previous study without affecting neuronal activity, suggesting that the activation of NMDA receptors through the glycine site by  -cycloserine could reverse the dysfunction in the coupling between neuronal activation and the rCBF response that is associated with a cholinergic blockade [ 43].	transcription
61040	3	335670	7	NULL	NULL	0	NULL	statement 2	Process		does not affect					neuronal activity	Process				NULL		0	NULL	NULL	NULL	gw60_brainres_832_1_118_s_98	10375657	-Cycloserine significantly recovered the rCBF response abolished by scopolamine in our previous study without affecting neuronal activity, suggesting that the activation of NMDA receptors through the glycine site by  -cycloserine could reverse the dysfunction in the coupling between neuronal activation and the rCBF response that is associated with a cholinergic blockade [ 43].	transcription
61041	4	335670	7	NULL	NULL	0	NULL	cycloserine	Chemical		activate					NMDA receptors	GP		glycine site		NULL		0	NULL	NULL	NULL	gw60_brainres_832_1_118_s_98	10375657	-Cycloserine significantly recovered the rCBF response abolished by scopolamine in our previous study without affecting neuronal activity, suggesting that the activation of NMDA receptors through the glycine site by  -cycloserine could reverse the dysfunction in the coupling between neuronal activation and the rCBF response that is associated with a cholinergic blockade [ 43].	transcription
61042	5	335670	7	NULL	NULL	0	NULL	neuronal activation	Process		coupled to					 rCBF response	Process				NULL		0	NULL	NULL	NULL	gw60_brainres_832_1_118_s_98	10375657	-Cycloserine significantly recovered the rCBF response abolished by scopolamine in our previous study without affecting neuronal activity, suggesting that the activation of NMDA receptors through the glycine site by  -cycloserine could reverse the dysfunction in the coupling between neuronal activation and the rCBF response that is associated with a cholinergic blockade [ 43].	transcription
61043	6	335670	7	NULL	NULL	0	NULL	statement 5	Process		associated with					choline	Chemical	blockade of			NULL		0	NULL	NULL	NULL	gw60_brainres_832_1_118_s_98	10375657	-Cycloserine significantly recovered the rCBF response abolished by scopolamine in our previous study without affecting neuronal activity, suggesting that the activation of NMDA receptors through the glycine site by  -cycloserine could reverse the dysfunction in the coupling between neuronal activation and the rCBF response that is associated with a cholinergic blockade [ 43].	transcription
61044	7	335670	7	NULL	NULL	0	NULL	statement 4	Process		reverse					statement 5	Process	dysfunction in			NULL		NULL	NULL	NULL	NULL	gw60_brainres_832_1_118_s_98	10375657	-Cycloserine significantly recovered the rCBF response abolished by scopolamine in our previous study without affecting neuronal activity, suggesting that the activation of NMDA receptors through the glycine site by  -cycloserine could reverse the dysfunction in the coupling between neuronal activation and the rCBF response that is associated with a cholinergic blockade [ 43].	transcription
61045	1	335671	7	NULL	NULL	0	NULL	NMDA	GP		stimulate					GABA	Chemical				NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_106_s_252	10536266	The difference in sensitivity between NMDA-stimulated [14]GABA and [3]ACh release to the NMDA antagonists, PCP, MK801 and mecamylamine, and to the glycine antagonists, CNQX, DNQX and 7-chlorokynurenic acid, might result from a difference in the subunit composition of the NMDA receptors found on cholinergic and on GABAergic neurons.	transcription
61046	2	335671	7	NULL	NULL	0	NULL	PCP	Chemical		release					ACh	Chemical				NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_106_s_252	10536266	The difference in sensitivity between NMDA-stimulated [14]GABA and [3]ACh release to the NMDA antagonists, PCP, MK801 and mecamylamine, and to the glycine antagonists, CNQX, DNQX and 7-chlorokynurenic acid, might result from a difference in the subunit composition of the NMDA receptors found on cholinergic and on GABAergic neurons.	transcription
61047	3	335671	7	NULL	NULL	0	NULL	MK801	Chemical		release from					ACh	Chemical				NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_106_s_252	10536266	The difference in sensitivity between NMDA-stimulated [14]GABA and [3]ACh release to the NMDA antagonists, PCP, MK801 and mecamylamine, and to the glycine antagonists, CNQX, DNQX and 7-chlorokynurenic acid, might result from a difference in the subunit composition of the NMDA receptors found on cholinergic and on GABAergic neurons.	transcription
61048	4	335671	7	NULL	NULL	0	NULL	mecamylamine	Chemical		release					ACh	Chemical				NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_106_s_252	10536266	The difference in sensitivity between NMDA-stimulated [14]GABA and [3]ACh release to the NMDA antagonists, PCP, MK801 and mecamylamine, and to the glycine antagonists, CNQX, DNQX and 7-chlorokynurenic acid, might result from a difference in the subunit composition of the NMDA receptors found on cholinergic and on GABAergic neurons.	transcription
61049	5	335671	7	NULL	NULL	0	NULL	CNQX	Chemical		release					ACh	Chemical				NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_106_s_252	10536266	The difference in sensitivity between NMDA-stimulated [14]GABA and [3]ACh release to the NMDA antagonists, PCP, MK801 and mecamylamine, and to the glycine antagonists, CNQX, DNQX and 7-chlorokynurenic acid, might result from a difference in the subunit composition of the NMDA receptors found on cholinergic and on GABAergic neurons.	transcription
61050	6	335671	7	NULL	NULL	0	NULL	DNQX	Chemical		release					ACh	Chemical				NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_106_s_252	10536266	The difference in sensitivity between NMDA-stimulated [14]GABA and [3]ACh release to the NMDA antagonists, PCP, MK801 and mecamylamine, and to the glycine antagonists, CNQX, DNQX and 7-chlorokynurenic acid, might result from a difference in the subunit composition of the NMDA receptors found on cholinergic and on GABAergic neurons.	transcription
61051	7	335671	7	NULL	NULL	0	NULL	7-chlorokynurenic acid	Chemical		release					ACh	Chemical				NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_106_s_252	10536266	The difference in sensitivity between NMDA-stimulated [14]GABA and [3]ACh release to the NMDA antagonists, PCP, MK801 and mecamylamine, and to the glycine antagonists, CNQX, DNQX and 7-chlorokynurenic acid, might result from a difference in the subunit composition of the NMDA receptors found on cholinergic and on GABAergic neurons.	transcription
61052	8	335671	7	NULL	NULL	0	NULL	NMDA receptor	GP	cholinergic neuron	differs from			subunit		NMDA receptor	GP	GABAergic neuron	subunit		NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_106_s_252	10536266	The difference in sensitivity between NMDA-stimulated [14]GABA and [3]ACh release to the NMDA antagonists, PCP, MK801 and mecamylamine, and to the glycine antagonists, CNQX, DNQX and 7-chlorokynurenic acid, might result from a difference in the subunit composition of the NMDA receptors found on cholinergic and on GABAergic neurons.	transcription
61053	9	335671	7	NULL	NULL	0	NULL	statement 1	Process	sensitivity of	differs with					statement 2	Process	sensitivity of			NULL		NULL	NULL	NULL	NULL	gw60_brainres_844_1_106_s_252	10536266	The difference in sensitivity between NMDA-stimulated [14]GABA and [3]ACh release to the NMDA antagonists, PCP, MK801 and mecamylamine, and to the glycine antagonists, CNQX, DNQX and 7-chlorokynurenic acid, might result from a difference in the subunit composition of the NMDA receptors found on cholinergic and on GABAergic neurons.	transcription
61054	10	335671	7	NULL	NULL	0	NULL	statement 1	Process	sensitivity of	differs with					statement 3	Process	sensitivity of			NULL		NULL	NULL	NULL	NULL	gw60_brainres_844_1_106_s_252	10536266	The difference in sensitivity between NMDA-stimulated [14]GABA and [3]ACh release to the NMDA antagonists, PCP, MK801 and mecamylamine, and to the glycine antagonists, CNQX, DNQX and 7-chlorokynurenic acid, might result from a difference in the subunit composition of the NMDA receptors found on cholinergic and on GABAergic neurons.	transcription
61055	11	335671	7	NULL	NULL	0	NULL	statement 1	Process	sensitivity of	differs with					statement 4	Process	sensitivity of			NULL		NULL	NULL	NULL	NULL	gw60_brainres_844_1_106_s_252	10536266	The difference in sensitivity between NMDA-stimulated [14]GABA and [3]ACh release to the NMDA antagonists, PCP, MK801 and mecamylamine, and to the glycine antagonists, CNQX, DNQX and 7-chlorokynurenic acid, might result from a difference in the subunit composition of the NMDA receptors found on cholinergic and on GABAergic neurons.	transcription
61056	12	335671	7	NULL	NULL	0	NULL	statement 1	Process	sensitivity of	differs with					statement 5	Process	sensitivity of			NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_106_s_252	10536266	The difference in sensitivity between NMDA-stimulated [14]GABA and [3]ACh release to the NMDA antagonists, PCP, MK801 and mecamylamine, and to the glycine antagonists, CNQX, DNQX and 7-chlorokynurenic acid, might result from a difference in the subunit composition of the NMDA receptors found on cholinergic and on GABAergic neurons.	transcription
61057	13	335671	7	NULL	NULL	0	NULL	statement 1	Process	sensitivity of	differs with					statement 6	Process	sensitivity of			NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_106_s_252	10536266	The difference in sensitivity between NMDA-stimulated [14]GABA and [3]ACh release to the NMDA antagonists, PCP, MK801 and mecamylamine, and to the glycine antagonists, CNQX, DNQX and 7-chlorokynurenic acid, might result from a difference in the subunit composition of the NMDA receptors found on cholinergic and on GABAergic neurons.	transcription
61058	14	335671	7	NULL	NULL	0	NULL	statement 1	Process	sensitivity of	differs with					statement 7	Process	sensitivity of			NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_106_s_252	10536266	The difference in sensitivity between NMDA-stimulated [14]GABA and [3]ACh release to the NMDA antagonists, PCP, MK801 and mecamylamine, and to the glycine antagonists, CNQX, DNQX and 7-chlorokynurenic acid, might result from a difference in the subunit composition of the NMDA receptors found on cholinergic and on GABAergic neurons.	transcription
61059	15	335671	7	NULL	NULL	0	NULL	statement 9	Process		because of					statement 8	Process				NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_106_s_252	10536266	The difference in sensitivity between NMDA-stimulated [14]GABA and [3]ACh release to the NMDA antagonists, PCP, MK801 and mecamylamine, and to the glycine antagonists, CNQX, DNQX and 7-chlorokynurenic acid, might result from a difference in the subunit composition of the NMDA receptors found on cholinergic and on GABAergic neurons.	transcription
61060	16	335671	7	NULL	NULL	0	NULL	statement 10	Process		because of					statement 8	Process				NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_106_s_252	10536266	The difference in sensitivity between NMDA-stimulated [14]GABA and [3]ACh release to the NMDA antagonists, PCP, MK801 and mecamylamine, and to the glycine antagonists, CNQX, DNQX and 7-chlorokynurenic acid, might result from a difference in the subunit composition of the NMDA receptors found on cholinergic and on GABAergic neurons.	transcription
61061	17	335671	7	NULL	NULL	0	NULL	statement 11	Process		because of					statement 8	Process				NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_106_s_252	10536266	The difference in sensitivity between NMDA-stimulated [14]GABA and [3]ACh release to the NMDA antagonists, PCP, MK801 and mecamylamine, and to the glycine antagonists, CNQX, DNQX and 7-chlorokynurenic acid, might result from a difference in the subunit composition of the NMDA receptors found on cholinergic and on GABAergic neurons.	transcription
61062	18	335671	7	NULL	NULL	0	NULL	statement 12	Process		because of					statement 8	Process				NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_106_s_252	10536266	The difference in sensitivity between NMDA-stimulated [14]GABA and [3]ACh release to the NMDA antagonists, PCP, MK801 and mecamylamine, and to the glycine antagonists, CNQX, DNQX and 7-chlorokynurenic acid, might result from a difference in the subunit composition of the NMDA receptors found on cholinergic and on GABAergic neurons.	transcription
61063	19	335671	7	NULL	NULL	0	NULL	statement 13	Process		because of					statement 8	Process				NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_106_s_252	10536266	The difference in sensitivity between NMDA-stimulated [14]GABA and [3]ACh release to the NMDA antagonists, PCP, MK801 and mecamylamine, and to the glycine antagonists, CNQX, DNQX and 7-chlorokynurenic acid, might result from a difference in the subunit composition of the NMDA receptors found on cholinergic and on GABAergic neurons.	transcription
61064	20	335671	7	NULL	NULL	0	NULL	statement 14	Process		because of					statement 8	Process				NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_106_s_252	10536266	The difference in sensitivity between NMDA-stimulated [14]GABA and [3]ACh release to the NMDA antagonists, PCP, MK801 and mecamylamine, and to the glycine antagonists, CNQX, DNQX and 7-chlorokynurenic acid, might result from a difference in the subunit composition of the NMDA receptors found on cholinergic and on GABAergic neurons.	transcription
61065	21	335671	7	NULL	NULL	0	NULL	PCP	Chemical		is a type of					NMDA antagonist	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_brainres_844_1_106_s_252	10536266	The difference in sensitivity between NMDA-stimulated [14]GABA and [3]ACh release to the NMDA antagonists, PCP, MK801 and mecamylamine, and to the glycine antagonists, CNQX, DNQX and 7-chlorokynurenic acid, might result from a difference in the subunit composition of the NMDA receptors found on cholinergic and on GABAergic neurons.	transcription
61066	22	335671	7	NULL	NULL	0	NULL	MK801	Chemical		is a type of					NMDA antagonist	Chemical				NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_106_s_252	10536266	The difference in sensitivity between NMDA-stimulated [14]GABA and [3]ACh release to the NMDA antagonists, PCP, MK801 and mecamylamine, and to the glycine antagonists, CNQX, DNQX and 7-chlorokynurenic acid, might result from a difference in the subunit composition of the NMDA receptors found on cholinergic and on GABAergic neurons.	transcription
61067	23	335671	7	NULL	NULL	0	NULL	mecamylamine	Chemical		is a type of					NMDA antagonist	Chemical				NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_106_s_252	10536266	The difference in sensitivity between NMDA-stimulated [14]GABA and [3]ACh release to the NMDA antagonists, PCP, MK801 and mecamylamine, and to the glycine antagonists, CNQX, DNQX and 7-chlorokynurenic acid, might result from a difference in the subunit composition of the NMDA receptors found on cholinergic and on GABAergic neurons.	transcription
61068	24	335671	7	NULL	NULL	0	NULL	CNQX	Chemical		is a type of					NMDA antagonist	Chemical				NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_106_s_252	10536266	The difference in sensitivity between NMDA-stimulated [14]GABA and [3]ACh release to the NMDA antagonists, PCP, MK801 and mecamylamine, and to the glycine antagonists, CNQX, DNQX and 7-chlorokynurenic acid, might result from a difference in the subunit composition of the NMDA receptors found on cholinergic and on GABAergic neurons.	transcription
61069	25	335671	7	NULL	NULL	0	NULL	DNQX	Chemical		is a type of					NMDA antagonist	Chemical				NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_106_s_252	10536266	The difference in sensitivity between NMDA-stimulated [14]GABA and [3]ACh release to the NMDA antagonists, PCP, MK801 and mecamylamine, and to the glycine antagonists, CNQX, DNQX and 7-chlorokynurenic acid, might result from a difference in the subunit composition of the NMDA receptors found on cholinergic and on GABAergic neurons.	transcription
61070	26	335671	7	NULL	NULL	0	NULL	7-chlorokynurenic acid	Chemical		is a type of					NMDA antagonist	Chemical				NULL		0	NULL	NULL	NULL	gw60_brainres_844_1_106_s_252	10536266	The difference in sensitivity between NMDA-stimulated [14]GABA and [3]ACh release to the NMDA antagonists, PCP, MK801 and mecamylamine, and to the glycine antagonists, CNQX, DNQX and 7-chlorokynurenic acid, might result from a difference in the subunit composition of the NMDA receptors found on cholinergic and on GABAergic neurons.	transcription
56506	1	335672	5	NULL	NULL	0	NULL	heme			stimulates					globin		synthesis of			NULL		0	NULL	NULL	NULL	gw60_jlipidres_40_7_1222_s_271	10393207	The stimulation of globin synthesis by heme.	transcription
61071	1	335672	7	NULL	NULL	0	NULL	heme	Chemical		stimulate					globin	GP	synthesis of			NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_40_7_1222_s_271	10393207	The stimulation of globin synthesis by heme.	transcription
61072	1	335673	7	NULL	NULL	0	NULL	globin	GP		interacts with					heme	Chemical				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1749_2_148_s_84	15927874	Dynamics of globin and the heme-globin interaction,  J. Mol.	transcription
56507	1	335674	5	NULL	NULL	0	NULL	heme			bind					globin chains		nascent			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10646_s_100	9099713	On the grounds of these data we suggest that heme binding to the nascent globin chains can be used as a test of cotranslational folding of globins.	transcription
61073	1	335674	7	NULL	NULL	0	NULL	heme	Chemical		bind					globin chains	GP	nascent			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10646_s_100	9099713	On the grounds of these data we suggest that heme binding to the nascent globin chains can be used as a test of cotranslational folding of globins.	transcription
56508	1	335675	5	NULL	NULL	0	NULL	heme			induces					beta-globin gene		transcription of			NULL		0	NULL	NULL	NULL	gw70_embo_23_13_2544_s_34	15175654	Importantly, heme induces transcription of the beta-globin gene ( ).	transcription
61074	1	335675	7	NULL	NULL	0	NULL	heme	Chemical		induce					beta-globin gene	GP	transcription of			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_13_2544_s_34	15175654	Importantly, heme induces transcription of the beta-globin gene ( ).	transcription
56509	1	335676	5	NULL	NULL	0	NULL	HRI			regulates					alpha-globin		synthesis of			NULL		0	NULL	NULL	NULL	gw60_embo_20_23_6909_s_251	11726526	( A) Regulation of alpha- and beta-globin synthesis by HRI and heme.	transcription
56510	2	335676	5	NULL	NULL	0	NULL	HRI			regulates					beta-globin		synthesis of			NULL		0	NULL	NULL	NULL	gw60_embo_20_23_6909_s_251	11726526	( A) Regulation of alpha- and beta-globin synthesis by HRI and heme.	transcription
56511	3	335676	5	NULL	NULL	0	NULL	heme			regulates					alpha-globin		synthesis of			NULL		0	NULL	NULL	NULL	gw60_embo_20_23_6909_s_251	11726526	( A) Regulation of alpha- and beta-globin synthesis by HRI and heme.	transcription
56512	4	335676	5	NULL	NULL	0	NULL	heme			regulates					beta-globin		synthesis of			NULL		0	NULL	NULL	NULL	gw60_embo_20_23_6909_s_251	11726526	( A) Regulation of alpha- and beta-globin synthesis by HRI and heme.	transcription
61075	1	335676	7	NULL	NULL	0	NULL	HRI	GP		regulate					alpha-globin	GP	synthesis of			NULL		0	NULL	NULL	NULL	gw60_embo_20_23_6909_s_251	11726526	( A) Regulation of alpha- and beta-globin synthesis by HRI and heme.	transcription
61076	2	335676	7	NULL	NULL	0	NULL	HRI	GP		regulate					beta-globin	GP	synthesis of			NULL		0	NULL	NULL	NULL	gw60_embo_20_23_6909_s_251	11726526	( A) Regulation of alpha- and beta-globin synthesis by HRI and heme.	transcription
61077	3	335676	7	NULL	NULL	0	NULL	heme	Chemical		regulate					alpha-globin	GP	synthesis of			NULL		0	NULL	NULL	NULL	gw60_embo_20_23_6909_s_251	11726526	( A) Regulation of alpha- and beta-globin synthesis by HRI and heme.	transcription
61078	4	335676	7	NULL	NULL	0	NULL	heme	Chemical		regulate					beta-globin	GP	synthesis of			NULL		0	NULL	NULL	NULL	gw60_embo_20_23_6909_s_251	11726526	( A) Regulation of alpha- and beta-globin synthesis by HRI and heme.	transcription
56513	1	335677	5	NULL	NULL	0	NULL	AHSP			bind					alpha-globin					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_43_40602_s_234	12192002	B, AHSP binds alpha-globin in the absence of heme.	transcription
56514	2	335677	5	NULL	NULL	0	NULL	statement 1			in absence of					heme					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_43_40602_s_234	12192002	B, AHSP binds alpha-globin in the absence of heme.	transcription
61079	1	335677	7	NULL	NULL	0	NULL	AHSP	GP		bind					alpha-globin	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_43_40602_s_234	12192002	B, AHSP binds alpha-globin in the absence of heme.	transcription
61080	2	335677	7	NULL	NULL	0	NULL	statement 1	Process		in the absence of					heme	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_43_40602_s_234	12192002	B, AHSP binds alpha-globin in the absence of heme.	transcription
61081	1	335678	7	NULL	NULL	0	NULL	Heme	Chemical		regulates					kinase	GP				NULL		0	NULL	NULL	NULL	gw70_jclininvest_114_10_1457_s_272	15545996	Heme-regulated kinase inhibits globin translation when heme availability is limited ( ).	transcription
61082	2	335678	7	NULL	NULL	0	NULL	statement 1	Process		inhibit					globin	GP	translation of			NULL		0	NULL	NULL	NULL	gw70_jclininvest_114_10_1457_s_272	15545996	Heme-regulated kinase inhibits globin translation when heme availability is limited ( ).	transcription
61083	3	335678	7	NULL	NULL	0	NULL	statement 1	Process		occur upon					heme	Chemical	limited availability of			NULL		0	NULL	NULL	NULL	gw70_jclininvest_114_10_1457_s_272	15545996	Heme-regulated kinase inhibits globin translation when heme availability is limited ( ).	transcription
56515	1	335679	5	NULL	NULL	0	NULL	globin			hydrolyzed by					THAP					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_37_28659_s_5	10896678	Hydrolysis of globin by THAP increased as increasing amounts of heme were added to globin, with maximum activation at a heme-to-globin 1:1 ratio.	transcription
61084	1	335679	7	NULL	NULL	0	NULL	THAP	GP		hydrolyze					globin	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_37_28659_s_5	10896678	Hydrolysis of globin by THAP increased as increasing amounts of heme were added to globin, with maximum activation at a heme-to-globin 1:1 ratio.	transcription
61085	1	335680	7	NULL	NULL	0	NULL	CooA	GP		does not resemble			heme-binding region of 					PAS domain		NULL		NULL	NULL	NULL	NULL	gw70_jbacteriol_186_5_1320_s_193	14973040	The heme-binding region of CooA does not resemble those of other common heme regions, such as the PAS domain ( ) or the heme domain found in globins ( ).	transcription
61086	2	335680	7	NULL	NULL	0	NULL	CooA	GP		does not resemble			heme-binding region of 		globins	GP		heme domain		NULL		0	NULL	NULL	NULL	gw70_jbacteriol_186_5_1320_s_193	14973040	The heme-binding region of CooA does not resemble those of other common heme regions, such as the PAS domain ( ) or the heme domain found in globins ( ).	transcription
56516	1	335681	5	NULL	NULL	0	NULL	globin		increase of;;synthesis of	leads to					globin		accumulation of			NULL	erythroid cells from iron-deficient HRI / mice	0	NULL	NULL	NULL	gw70_annurevnutr_24_0_105_s_479	15189115	However, in erythroid cells from iron-deficient HRI /  mice, a marked increase in both  - and  -globin synthesis led to accumulated globins  that were devoid of heme and aggregated within the erythrocytes and their precursors.	transcription
56517	2	335681	5	NULL	NULL	0	NULL	globin		accumulated	is devoid of					heme					NULL		0	NULL	NULL	NULL	gw70_annurevnutr_24_0_105_s_479	15189115	However, in erythroid cells from iron-deficient HRI /  mice, a marked increase in both  - and  -globin synthesis led to accumulated globins  that were devoid of heme and aggregated within the erythrocytes and their precursors.	transcription
56518	3	335681	5	NULL	NULL	0	NULL	statement 2			is aggregated within					erythrocytes					NULL		0	NULL	NULL	NULL	gw70_annurevnutr_24_0_105_s_479	15189115	However, in erythroid cells from iron-deficient HRI /  mice, a marked increase in both  - and  -globin synthesis led to accumulated globins  that were devoid of heme and aggregated within the erythrocytes and their precursors.	transcription
61087	1	335681	7	NULL	NULL	0	NULL	globin	GP	increase in synthesis of	leads to					globins	GP	accumulation of			NULL	erythroid cells from iron-deficient HRI / mice	0	NULL	NULL	NULL	gw70_annurevnutr_24_0_105_s_479	15189115	However, in erythroid cells from iron-deficient HRI /  mice, a marked increase in both  - and  -globin synthesis led to accumulated globins  that were devoid of heme and aggregated within the erythrocytes and their precursors.	transcription
61088	2	335681	7	NULL	NULL	0	NULL	globins	GP		devoid of					heme	Chemical				NULL		0	NULL	NULL	NULL	gw70_annurevnutr_24_0_105_s_479	15189115	However, in erythroid cells from iron-deficient HRI /  mice, a marked increase in both  - and  -globin synthesis led to accumulated globins  that were devoid of heme and aggregated within the erythrocytes and their precursors.	transcription
61089	3	335681	7	NULL	NULL	0	NULL	statement 2	Process		aggregates within					erythrocytes	Cell				NULL		0	NULL	NULL	NULL	gw70_annurevnutr_24_0_105_s_479	15189115	However, in erythroid cells from iron-deficient HRI /  mice, a marked increase in both  - and  -globin synthesis led to accumulated globins  that were devoid of heme and aggregated within the erythrocytes and their precursors.	transcription
66477	1	335682	7	NULL	NULL	0	NULL	HRI	GP		evolved from			NT-HBD		globin gene	GP			second exon of	NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1725_2_174_s_68	16109458	However, while the analyses suggest  that the NT-HBD of HRI may have evolved from the second exon of the  -globin gene    [12], the finding that His123 may be one of the axial heme-binding ligands   [17] suggests that the tertiary fold of the NT-HBD may be different from that of globin  chains, as H123 is predicted to be part of what would be equivalent to the H-helix of globins: a  helix located outside the heme-binding core of globins   [12].	transcription
66478	2	335682	7	NULL	NULL	0	NULL	His123	GP		is a type of					axial heme-binding ligands	GP				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1725_2_174_s_68	16109458	However, while the analyses suggest  that the NT-HBD of HRI may have evolved from the second exon of the  -globin gene    [12], the finding that His123 may be one of the axial heme-binding ligands   [17] suggests that the tertiary fold of the NT-HBD may be different from that of globin  chains, as H123 is predicted to be part of what would be equivalent to the H-helix of globins: a  helix located outside the heme-binding core of globins   [12].	transcription
66479	3	335682	7	NULL	NULL	0	NULL	HRI	GP		different from		may be	NT-HBD 		globin chains	GP				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1725_2_174_s_68	16109458	However, while the analyses suggest  that the NT-HBD of HRI may have evolved from the second exon of the  -globin gene    [12], the finding that His123 may be one of the axial heme-binding ligands   [17] suggests that the tertiary fold of the NT-HBD may be different from that of globin  chains, as H123 is predicted to be part of what would be equivalent to the H-helix of globins: a  helix located outside the heme-binding core of globins   [12].	transcription
66480	4	335682	7	NULL	NULL	0	NULL	H123	GP		is equivalent to					globins	GP	part of	H-helix of 		NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1725_2_174_s_68	16109458	However, while the analyses suggest  that the NT-HBD of HRI may have evolved from the second exon of the  -globin gene    [12], the finding that His123 may be one of the axial heme-binding ligands   [17] suggests that the tertiary fold of the NT-HBD may be different from that of globin  chains, as H123 is predicted to be part of what would be equivalent to the H-helix of globins: a  helix located outside the heme-binding core of globins   [12].	transcription
56664	1	335683	5	NULL	NULL	0	NULL	HRI			regulates					globin		synthesis of			NULL	reticulocytes	0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15752_s_17	14752110	HRI regulates globin synthesis in reticulocytes in response to heme availability.	transcription
56665	2	335683	5	NULL	NULL	0	NULL	statement 1			in response to					heme		availability of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15752_s_17	14752110	HRI regulates globin synthesis in reticulocytes in response to heme availability.	transcription
66481	1	335683	7	NULL	NULL	0	NULL	HRI 	GP		regulates					globin	GP	synthesis of			NULL	reticulocytes	0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15752_s_17	14752110	HRI regulates globin synthesis in reticulocytes in response to heme availability.	transcription
66482	2	335683	7	NULL	NULL	0	NULL	statement 1	Process		in response to					heme	GP	availability of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_16_15752_s_17	14752110	HRI regulates globin synthesis in reticulocytes in response to heme availability.	transcription
56666	1	335684	5	NULL	NULL	0	NULL	heme			bind					globin					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_22_22944_s_247	15016813	Remarkably, as in murine Ngb, the heme binds to the globin in two orientations in  Chironomus Hb ( ,  ).	transcription
56667	2	335684	5	NULL	NULL	0	NULL	statement 1			occurs in					Hb		Chironomus			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_22_22944_s_247	15016813	Remarkably, as in murine Ngb, the heme binds to the globin in two orientations in  Chironomus Hb ( ,  ).	transcription
56668	3	335684	5	NULL	NULL	0	NULL	statement 1			occurs in					Ngb		murine			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_22_22944_s_247	15016813	Remarkably, as in murine Ngb, the heme binds to the globin in two orientations in  Chironomus Hb ( ,  ).	transcription
66483	1	335684	7	NULL	NULL	0	NULL	heme	Chemical		bind					globin	GP				NULL	Chironomus Hb	0	NULL	NULL	NULL	gw70_jbiolchem_279_22_22944_s_247	15016813	Remarkably, as in murine Ngb, the heme binds to the globin in two orientations in  Chironomus Hb ( ,  ).	transcription
66484	2	335684	7	NULL	NULL	0	NULL	statement 1	Process		occur in					two orientations	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_22_22944_s_247	15016813	Remarkably, as in murine Ngb, the heme binds to the globin in two orientations in  Chironomus Hb ( ,  ).	transcription
66485	3	335684	7	NULL	NULL	0	NULL	Heme	Chemical		bind					globin	GP				NULL	murine Ngb	0	NULL	NULL	NULL	gw70_jbiolchem_279_22_22944_s_247	15016813	Remarkably, as in murine Ngb, the heme binds to the globin in two orientations in  Chironomus Hb ( ,  ).	transcription
56669	1	335685	5	NULL	NULL	0	NULL	Bach1			departs from					beta-Globin LCR					NULL		0	NULL	NULL	NULL	gw70_pnas_101_6_1461_s_179	14747657	Heme Induces the Departure of Bach1 from the beta-Globin LCR.	transcription
56670	2	335685	5	NULL	NULL	0	NULL	heme			induce					statement 1					NULL		0	NULL	NULL	NULL	gw70_pnas_101_6_1461_s_179	14747657	Heme Induces the Departure of Bach1 from the beta-Globin LCR.	transcription
66486	1	335685	7	NULL	NULL	0	NULL	Bach1	GP		depart from					beta-Globin	GP		LCR		NULL		0	NULL	NULL	NULL	gw70_pnas_101_6_1461_s_179	14747657	Heme Induces the Departure of Bach1 from the beta-Globin LCR.	transcription
66487	2	335685	7	NULL	NULL	0	NULL	Heme	Chemical		induce					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_101_6_1461_s_179	14747657	Heme Induces the Departure of Bach1 from the beta-Globin LCR.	transcription
56671	1	335686	5	NULL	NULL	0	NULL	globin			undergoes					translation					NULL		0	NULL	NULL	NULL	gw60_embo_20_23_6909_s_235	11726526	The lack of HRI relieves the normal feedback regulation of globin translation in heme deficiency.	transcription
56672	2	335686	5	NULL	NULL	0	NULL	statement 1			in deficiency of					heme					NULL		0	NULL	NULL	NULL	gw60_embo_20_23_6909_s_235	11726526	The lack of HRI relieves the normal feedback regulation of globin translation in heme deficiency.	transcription
56673	3	335686	5	NULL	NULL	0	NULL	HRI		absence of	relieves					statement 1		normal feedback regulation of			NULL		0	NULL	NULL	NULL	gw60_embo_20_23_6909_s_235	11726526	The lack of HRI relieves the normal feedback regulation of globin translation in heme deficiency.	transcription
66488	1	335686	7	NULL	NULL	0	NULL	HRI	GP	lack of	relieves					globin translation	Process	normal feedback regulation of			NULL		0	NULL	NULL	NULL	gw60_embo_20_23_6909_s_235	11726526	The lack of HRI relieves the normal feedback regulation of globin translation in heme deficiency.	transcription
66489	2	335686	7	NULL	NULL	0	NULL	statement 1	Process		occurs in					heme deficiency	MedicalFinding				NULL		0	NULL	NULL	NULL	gw60_embo_20_23_6909_s_235	11726526	The lack of HRI relieves the normal feedback regulation of globin translation in heme deficiency.	transcription
56674	1	335687	5	NULL	NULL	0	NULL	HRI			is a feedback inhibitor of					globin		synthesis of			NULL		0	NULL	NULL	NULL	gw60_embo_20_23_6909_s_245	11726526	HRI serves as a feedback inhibitor of globin synthesis by sensing heme.	transcription
56675	2	335687	5	NULL	NULL	0	NULL	statement 1			occurs by					heme		sensing of			NULL		0	NULL	NULL	NULL	gw60_embo_20_23_6909_s_245	11726526	HRI serves as a feedback inhibitor of globin synthesis by sensing heme.	transcription
66490	1	335687	7	NULL	NULL	0	NULL	HRI	GP		is a feedback inhibitor of					globin synthesis	Process				NULL		0	NULL	NULL	NULL	gw60_embo_20_23_6909_s_245	11726526	HRI serves as a feedback inhibitor of globin synthesis by sensing heme.	transcription
66491	2	335687	7	NULL	NULL	0	NULL	statement 1	Process		occur by 					heme	Chemical	sensing			NULL		0	NULL	NULL	NULL	gw60_embo_20_23_6909_s_245	11726526	HRI serves as a feedback inhibitor of globin synthesis by sensing heme.	transcription
56676	1	335688	5	NULL	NULL	0	NULL	heme			bind					globin					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_640_s_301	9925594	The association rate constant for heme binding to globin is independent of protein structure.	transcription
66492	1	335688	7	NULL	NULL	0	NULL	heme	Chemical		bind					globin	GP				NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_640_s_301	9925594	The association rate constant for heme binding to globin is independent of protein structure.	transcription
56677	1	335689	5	NULL	NULL	0	NULL	alpha-globin			is not required for			heme group		AHSP		interaction with			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_43_40602_s_33	12192002	In addition, we find that the heme group of alpha-globin is not required for AHSP interaction.	transcription
66493	1	335689	7	NULL	NULL	0	NULL	 alpha-globin	GP		is not required for			heme group		AHSP	GP	interaction of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_43_40602_s_33	12192002	In addition, we find that the heme group of alpha-globin is not required for AHSP interaction.	transcription
56678	1	335690	5	NULL	NULL	0	NULL	globin			contains								heme-binding domain		NULL		0	NULL	NULL	NULL	gw70_jneurosci_23_28_9418_s_323	14561870	Globins contain a heme-binding domain and participate in diverse processes such as oxygen transport, oxygen storage, and nitric oxide detoxification.	transcription
56679	2	335690	5	NULL	NULL	0	NULL	statement 1			participates in					oxygen		transport of			NULL		0	NULL	NULL	NULL	gw70_jneurosci_23_28_9418_s_323	14561870	Globins contain a heme-binding domain and participate in diverse processes such as oxygen transport, oxygen storage, and nitric oxide detoxification.	transcription
56680	3	335690	5	NULL	NULL	0	NULL	statement 1			participates in					oxygen		storage of			NULL		0	NULL	NULL	NULL	gw70_jneurosci_23_28_9418_s_323	14561870	Globins contain a heme-binding domain and participate in diverse processes such as oxygen transport, oxygen storage, and nitric oxide detoxification.	transcription
56681	4	335690	5	NULL	NULL	0	NULL	statement 1			participates in					nitric oxide		detoxification of			NULL		0	NULL	NULL	NULL	gw70_jneurosci_23_28_9418_s_323	14561870	Globins contain a heme-binding domain and participate in diverse processes such as oxygen transport, oxygen storage, and nitric oxide detoxification.	transcription
66494	1	335690	7	NULL	NULL	0	NULL	Globins	GP		contains					heme-binding domain	GP				NULL		0	NULL	NULL	NULL	gw70_jneurosci_23_28_9418_s_323	14561870	Globins contain a heme-binding domain and participate in diverse processes such as oxygen transport, oxygen storage, and nitric oxide detoxification.	transcription
66495	2	335690	7	NULL	NULL	0	NULL	Globins	GP		participate in					oxygen transport	Process				NULL		0	NULL	NULL	NULL	gw70_jneurosci_23_28_9418_s_323	14561870	Globins contain a heme-binding domain and participate in diverse processes such as oxygen transport, oxygen storage, and nitric oxide detoxification.	transcription
66496	3	335690	7	NULL	NULL	0	NULL	globins	GP		participate in					oxygen storage	Process				NULL		0	NULL	NULL	NULL	gw70_jneurosci_23_28_9418_s_323	14561870	Globins contain a heme-binding domain and participate in diverse processes such as oxygen transport, oxygen storage, and nitric oxide detoxification.	transcription
66497	4	335690	7	NULL	NULL	0	NULL	Globins	GP		participate in					nitric oxide detoxification	Process				NULL		0	NULL	NULL	NULL	gw70_jneurosci_23_28_9418_s_323	14561870	Globins contain a heme-binding domain and participate in diverse processes such as oxygen transport, oxygen storage, and nitric oxide detoxification.	transcription
56682	1	335691	5	NULL	NULL	0	NULL	heme			induce					beta-globin gene		expression of			NULL	erythroid cells	0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_121	14660636	Thus, heme induces the expression of the beta-globin gene by stimulating the enhancer activity of the beta-globin LCR in erythroid cells.	transcription
56683	2	335691	5	NULL	NULL	0	NULL	heme			stimulates					beta-globin LCR		activity of		enhancer	NULL	erythroid cells	0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_121	14660636	Thus, heme induces the expression of the beta-globin gene by stimulating the enhancer activity of the beta-globin LCR in erythroid cells.	transcription
56684	3	335691	5	NULL	NULL	0	NULL	statement 2			leads to					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_121	14660636	Thus, heme induces the expression of the beta-globin gene by stimulating the enhancer activity of the beta-globin LCR in erythroid cells.	transcription
66498	1	335691	7	NULL	NULL	0	NULL	heme	Chemical		induce					beta-globin gene	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_121	14660636	Thus, heme induces the expression of the beta-globin gene by stimulating the enhancer activity of the beta-globin LCR in erythroid cells.	transcription
66499	2	335691	7	NULL	NULL	NULL	NULL	statement 1	Process		occur by 					beta-globin	GP	stimulating;;enhancer activity of	LCR		NULL	erythroid cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_121	14660636	Thus, heme induces the expression of the beta-globin gene by stimulating the enhancer activity of the beta-globin LCR in erythroid cells.	transcription
66500	1	335692	7	NULL	NULL	0	NULL	Mutations	Process		result in					globin 	GP	instability of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_43_26931_s_26	8900178	Mutations that result in globin instability either affect structure of globin and heme subunit or hemoglobin tetramer.	transcription
66501	2	335692	7	NULL	NULL	0	NULL	statement 1	Process		affect					globin	GP	structure of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_43_26931_s_26	8900178	Mutations that result in globin instability either affect structure of globin and heme subunit or hemoglobin tetramer.	transcription
66502	3	335692	7	NULL	NULL	NULL	NULL	statement 1	Process		affect					heme subunit	Chemical	structure of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_43_26931_s_26	8900178	Mutations that result in globin instability either affect structure of globin and heme subunit or hemoglobin tetramer.	transcription
66503	4	335692	7	NULL	NULL	0	NULL	statement 1	Process		affect					hemoglobin tetramer	GP	structure of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_43_26931_s_26	8900178	Mutations that result in globin instability either affect structure of globin and heme subunit or hemoglobin tetramer.	transcription
66504	5	335692	7	NULL	NULL	0	NULL	statement 2	Process		is an alternative to					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_43_26931_s_26	8900178	Mutations that result in globin instability either affect structure of globin and heme subunit or hemoglobin tetramer.	transcription
66505	6	335692	7	NULL	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_43_26931_s_26	8900178	Mutations that result in globin instability either affect structure of globin and heme subunit or hemoglobin tetramer.	transcription
56685	1	335693	5	NULL	NULL	0	NULL	heme		synthesis of	is coupled with					beta-globin mRNA		transcription of			NULL		0	NULL	NULL	NULL	gw70_embo_23_13_2544_s_259	15175654	In this  view, synthesis of heme is coupled with transcription of beta-globin mRNA by the heme response of Bach1.	transcription
56686	2	335693	5	NULL	NULL	0	NULL	Bach1		heme response of	is required for					statement 1					NULL		0	NULL	NULL	NULL	gw70_embo_23_13_2544_s_259	15175654	In this  view, synthesis of heme is coupled with transcription of beta-globin mRNA by the heme response of Bach1.	transcription
66506	1	335693	7	NULL	NULL	0	NULL	heme	Chemical	synthesis of	is coupled with					beta-globin mRNA	GP	transcription of			NULL		0	NULL	NULL	NULL	gw70_embo_23_13_2544_s_259	15175654	In this  view, synthesis of heme is coupled with transcription of beta-globin mRNA by the heme response of Bach1.	transcription
66507	2	335693	7	NULL	NULL	0	NULL	statement 1	Process		occur by					Bach1	GP	heme response of			NULL		0	NULL	NULL	NULL	gw70_embo_23_13_2544_s_259	15175654	In this  view, synthesis of heme is coupled with transcription of beta-globin mRNA by the heme response of Bach1.	transcription
56687	1	335694	5	NULL	NULL	0	NULL	globin mRNA		translation of	is controlled by					heme					NULL	mammalian reticulocytes	0	NULL	NULL	NULL	gw70_jbacteriol_187_15_5084_s_20	16030200	Translation of globin mRNA in mammalian reticulocytes is controlled by heme via the heme-controlled inhibitor ( ).	transcription
56688	2	335694	5	NULL	NULL	0	NULL	statement 1			via					heme-controlled inhibitor					NULL	mammalian reticulocytes	NULL	NULL	NULL	NULL	gw70_jbacteriol_187_15_5084_s_20	16030200	Translation of globin mRNA in mammalian reticulocytes is controlled by heme via the heme-controlled inhibitor ( ).	transcription
66508	1	335694	7	NULL	NULL	0	NULL	globin mRNA	GP	translation of	is controlled by					heme	Chemical				NULL	mammalian reticulocytes	0	NULL	NULL	NULL	gw70_jbacteriol_187_15_5084_s_20	16030200	Translation of globin mRNA in mammalian reticulocytes is controlled by heme via the heme-controlled inhibitor ( ).	transcription
66509	2	335694	7	NULL	NULL	0	NULL	statement 1	Process		via					heme-controlled inhibitor	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbacteriol_187_15_5084_s_20	16030200	Translation of globin mRNA in mammalian reticulocytes is controlled by heme via the heme-controlled inhibitor ( ).	transcription
56689	1	335695	5	NULL	NULL	0	NULL	HRI			is					Heme-regulated eukaryotic initiation factor (eIF)-2 kinase					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_99_s_3	12922173	Heme-regulated eukaryotic initiation factor (eIF)-2  kinase (HRI) regulates the synthesis of globin chains in reticulocytes with heme availability.	transcription
56690	2	335695	5	NULL	NULL	0	NULL	HRI			regulates					globin chains		synthesis of			NULL	reticulocytes with heme availability	0	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_99_s_3	12922173	Heme-regulated eukaryotic initiation factor (eIF)-2  kinase (HRI) regulates the synthesis of globin chains in reticulocytes with heme availability.	transcription
66510	1	335695	7	NULL	NULL	0	NULL	HRI	GP		regulate 					globin chains	GP	synthesis of			NULL	reticulocytes	0	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_99_s_3	12922173	Heme-regulated eukaryotic initiation factor (eIF)-2  kinase (HRI) regulates the synthesis of globin chains in reticulocytes with heme availability.	transcription
66511	2	335695	7	NULL	NULL	0	NULL	statement 1	Process		occur with					heme 	Chemical	availability of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_99_s_3	12922173	Heme-regulated eukaryotic initiation factor (eIF)-2  kinase (HRI) regulates the synthesis of globin chains in reticulocytes with heme availability.	transcription
66512	3	335695	7	NULL	NULL	NULL	NULL	Heme-regulated eukaryotic initiation factor (eIF)-2 kinase	GP		is a type of					HRI	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_99_s_3	12922173	Heme-regulated eukaryotic initiation factor (eIF)-2  kinase (HRI) regulates the synthesis of globin chains in reticulocytes with heme availability.	transcription
66513	1	335696	7	NULL	NULL	0	NULL	heme binding module	GP		regulate					heme binding structure	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_17_12438_s_33	10777528	This structural conversion in the Mbalpha(HBM)-globin clearly demonstrated that the heme binding structure is regulated by the heme binding module.	transcription
56691	2	335697	5	NULL	NULL	0	NULL	linkers			does not bind					statement 1					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_47_29999_s_189	8939946	We conclude that the linkers do not bind heme under conditions where heme is not lost by the globin chains.	transcription
56692	1	335697	5	NULL	NULL	0	NULL	heme			is not lost by					globin chains					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_47_29999_s_189	8939946	We conclude that the linkers do not bind heme under conditions where heme is not lost by the globin chains.	transcription
66514	1	335697	7	NULL	NULL	0	NULL	linkers	GP		does not bind					heme	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_47_29999_s_189	8939946	We conclude that the linkers do not bind heme under conditions where heme is not lost by the globin chains.	transcription
66515	2	335697	7	NULL	NULL	0	NULL	heme	Chemical		is not lost by					globin chain	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_47_29999_s_189	8939946	We conclude that the linkers do not bind heme under conditions where heme is not lost by the globin chains.	transcription
66516	3	335697	7	NULL	NULL	0	NULL	statement 1	Process		occur upon					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_47_29999_s_189	8939946	We conclude that the linkers do not bind heme under conditions where heme is not lost by the globin chains.	transcription
56693	1	335698	5	NULL	NULL	0	NULL	heme			regulates					globin gene		transcription of			NULL	erythroleukemia cells	0	NULL	NULL	NULL	abs-batch0600-0619_antioxid-redox-signal_8_1-2_16487039_s_1	16487039	Regulation of Globin Gene Transcription by Heme in Erythroleukemia Cells: Analysis of Putative Heme Regulatory Motifs in the p45 NF-E2 Transcription Factor..	transcription
66517	1	335698	7	NULL	NULL	NULL	NULL	Heme	Chemical		regulate					Globin gene	GP	transcription of			NULL	Erythroleukemia Cells	NULL	NULL	NULL	NULL	abs-batch0600-0619_antioxid-redox-signal_8_1-2_16487039_s_1	16487039	Regulation of Globin Gene Transcription by Heme in Erythroleukemia Cells: Analysis of Putative Heme Regulatory Motifs in the p45 NF-E2 Transcription Factor..	transcription
56694	1	335699	5	NULL	NULL	0	NULL	HRI			is					Heme-regulated eIF2alpha kinase					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_12_5205_s_255	15923635	Heme-regulated eIF2alpha kinase (HRI) phosphorylates and inactivates eukaryotic initiation factor 2alpha (eIF2alpha) in the absence of heme ( ), thereby coordinating heme and globin synthesis ( ).	transcription
56695	2	335699	5	NULL	NULL	0	NULL	eIF2alpha			is					eukaryotic initiation factor 2alpha					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_12_5205_s_255	15923635	Heme-regulated eIF2alpha kinase (HRI) phosphorylates and inactivates eukaryotic initiation factor 2alpha (eIF2alpha) in the absence of heme ( ), thereby coordinating heme and globin synthesis ( ).	transcription
56696	3	335699	5	NULL	NULL	0	NULL	HRI			phosphorylates					eIF2alpha					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_12_5205_s_255	15923635	Heme-regulated eIF2alpha kinase (HRI) phosphorylates and inactivates eukaryotic initiation factor 2alpha (eIF2alpha) in the absence of heme ( ), thereby coordinating heme and globin synthesis ( ).	transcription
56697	4	335699	5	NULL	NULL	0	NULL	statement 3			inactivates					eIF2alpha					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_12_5205_s_255	15923635	Heme-regulated eIF2alpha kinase (HRI) phosphorylates and inactivates eukaryotic initiation factor 2alpha (eIF2alpha) in the absence of heme ( ), thereby coordinating heme and globin synthesis ( ).	transcription
56698	5	335699	5	NULL	NULL	0	NULL	statement 3			in the absence of					heme					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_12_5205_s_255	15923635	Heme-regulated eIF2alpha kinase (HRI) phosphorylates and inactivates eukaryotic initiation factor 2alpha (eIF2alpha) in the absence of heme ( ), thereby coordinating heme and globin synthesis ( ).	transcription
56699	6	335699	5	NULL	NULL	0	NULL	statement 4			coordinates with					heme		synthesis of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_12_5205_s_255	15923635	Heme-regulated eIF2alpha kinase (HRI) phosphorylates and inactivates eukaryotic initiation factor 2alpha (eIF2alpha) in the absence of heme ( ), thereby coordinating heme and globin synthesis ( ).	transcription
56700	7	335699	5	NULL	NULL	0	NULL	statement 4			coordinates with					globin		synthesis of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_12_5205_s_255	15923635	Heme-regulated eIF2alpha kinase (HRI) phosphorylates and inactivates eukaryotic initiation factor 2alpha (eIF2alpha) in the absence of heme ( ), thereby coordinating heme and globin synthesis ( ).	transcription
66518	1	335699	7	NULL	NULL	NULL	NULL	HRI	GP		is					Heme-regulated eIF2alpha kinase	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_5205_s_255	15923635	Heme-regulated eIF2alpha kinase (HRI) phosphorylates and inactivates eukaryotic initiation factor 2alpha (eIF2alpha) in the absence of heme ( ), thereby coordinating heme and globin synthesis ( ).	transcription
66519	2	335699	7	NULL	NULL	NULL	NULL	HRI	GP		phosphorylates					eIF2alpha	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_5205_s_255	15923635	Heme-regulated eIF2alpha kinase (HRI) phosphorylates and inactivates eukaryotic initiation factor 2alpha (eIF2alpha) in the absence of heme ( ), thereby coordinating heme and globin synthesis ( ).	transcription
66520	3	335699	7	NULL	NULL	0	NULL	HRI	GP		inactivates					eIF2alpha	GP				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_12_5205_s_255	15923635	Heme-regulated eIF2alpha kinase (HRI) phosphorylates and inactivates eukaryotic initiation factor 2alpha (eIF2alpha) in the absence of heme ( ), thereby coordinating heme and globin synthesis ( ).	transcription
66521	4	335699	7	NULL	NULL	0	NULL	statement 2	Process		in the absence of					heme	Chemical				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_12_5205_s_255	15923635	Heme-regulated eIF2alpha kinase (HRI) phosphorylates and inactivates eukaryotic initiation factor 2alpha (eIF2alpha) in the absence of heme ( ), thereby coordinating heme and globin synthesis ( ).	transcription
66522	5	335699	7	NULL	NULL	0	NULL	statement 3	Process		in the absence of					heme	Chemical				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_12_5205_s_255	15923635	Heme-regulated eIF2alpha kinase (HRI) phosphorylates and inactivates eukaryotic initiation factor 2alpha (eIF2alpha) in the absence of heme ( ), thereby coordinating heme and globin synthesis ( ).	transcription
66523	6	335699	7	NULL	NULL	0	NULL	statement 2	Process		coordinate					heme synthesis	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_12_5205_s_255	15923635	Heme-regulated eIF2alpha kinase (HRI) phosphorylates and inactivates eukaryotic initiation factor 2alpha (eIF2alpha) in the absence of heme ( ), thereby coordinating heme and globin synthesis ( ).	transcription
66524	7	335699	7	NULL	NULL	0	NULL	statement 3	Process		coordinate					heme synthesis	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_12_5205_s_255	15923635	Heme-regulated eIF2alpha kinase (HRI) phosphorylates and inactivates eukaryotic initiation factor 2alpha (eIF2alpha) in the absence of heme ( ), thereby coordinating heme and globin synthesis ( ).	transcription
66525	8	335699	7	NULL	NULL	0	NULL	statement 2	Process		coordinate					globin synthesis	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_12_5205_s_255	15923635	Heme-regulated eIF2alpha kinase (HRI) phosphorylates and inactivates eukaryotic initiation factor 2alpha (eIF2alpha) in the absence of heme ( ), thereby coordinating heme and globin synthesis ( ).	transcription
66526	9	335699	7	NULL	NULL	0	NULL	statement 3	Process		coordinate					globin synthesis	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_12_5205_s_255	15923635	Heme-regulated eIF2alpha kinase (HRI) phosphorylates and inactivates eukaryotic initiation factor 2alpha (eIF2alpha) in the absence of heme ( ), thereby coordinating heme and globin synthesis ( ).	transcription
66528	10	335699	7	NULL	NULL	NULL	NULL	eIF2alpha	GP		is					eukaryotic initiation factor 2alpha	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_12_5205_s_255	15923635	Heme-regulated eIF2alpha kinase (HRI) phosphorylates and inactivates eukaryotic initiation factor 2alpha (eIF2alpha) in the absence of heme ( ), thereby coordinating heme and globin synthesis ( ).	transcription
56701	1	335700	5	NULL	NULL	0	NULL	N-RsbR		B. subtilis	is a member of					globins family					NULL		0	NULL	NULL	NULL	gw70_pnas_102_48_17320_s_230	16301540	It is thus possible that globins with functions other than binding of gaseous diatomic molecules are yet to be discovered and that N-RsbR of  B. subtilis is the first member to be described of what could prove to be a large family of globins that do not bind heme.	transcription
56702	2	335700	5	NULL	NULL	0	NULL	N-RsbR		B. subtilis	does not bind					heme					NULL		0	NULL	NULL	NULL	gw70_pnas_102_48_17320_s_230	16301540	It is thus possible that globins with functions other than binding of gaseous diatomic molecules are yet to be discovered and that N-RsbR of  B. subtilis is the first member to be described of what could prove to be a large family of globins that do not bind heme.	transcription
66529	1	335700	7	NULL	NULL	0	NULL	N-RsbR	GP	B. subtilis	belongs to					globin family	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_102_48_17320_s_230	16301540	It is thus possible that globins with functions other than binding of gaseous diatomic molecules are yet to be discovered and that N-RsbR of  B. subtilis is the first member to be described of what could prove to be a large family of globins that do not bind heme.	transcription
66530	2	335700	7	NULL	NULL	NULL	NULL	N-RsbR	GP	B.subtilis	does not bind					heme	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_48_17320_s_230	16301540	It is thus possible that globins with functions other than binding of gaseous diatomic molecules are yet to be discovered and that N-RsbR of  B. subtilis is the first member to be described of what could prove to be a large family of globins that do not bind heme.	transcription
56703	1	335701	5	NULL	NULL	0	NULL	heme			bind					globin					NULL		0	NULL	NULL	NULL	gw70_embo_22_8_1824_s_202	12682015	Also similar to TipAS antibiotic binding, heme  binding to globins induces the folding of additional alpha-helices that are in contact with the ligand ( ;   et al;   et al).	transcription
56704	2	335701	5	NULL	NULL	0	NULL	statement 1			induces					alpha-helices		folding of			NULL		0	NULL	NULL	NULL	gw70_embo_22_8_1824_s_202	12682015	Also similar to TipAS antibiotic binding, heme  binding to globins induces the folding of additional alpha-helices that are in contact with the ligand ( ;   et al;   et al).	transcription
66531	1	335701	7	NULL	NULL	0	NULL	heme	Chemical		bind					globin	GP				NULL		0	NULL	NULL	NULL	gw70_embo_22_8_1824_s_202	12682015	Also similar to TipAS antibiotic binding, heme  binding to globins induces the folding of additional alpha-helices that are in contact with the ligand ( ;   et al;   et al).	transcription
66532	2	335701	7	NULL	NULL	0	NULL	heme	Chemical		induce					alpha-helices	GP	folding of			NULL		0	NULL	NULL	NULL	gw70_embo_22_8_1824_s_202	12682015	Also similar to TipAS antibiotic binding, heme  binding to globins induces the folding of additional alpha-helices that are in contact with the ligand ( ;   et al;   et al).	transcription
66533	1	335702	7	NULL	NULL	0	NULL	heme	Chemical		bind								NTD		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_6778_s_12	14672943	His78 appears to play the primary role in the specific binding of heme to the NTD, acting analogously to the "`proximal histidine"` ligand of globins, while His123 appears to act as the "`distal"` heme ligand.	transcription
66534	2	335702	7	NULL	NULL	0	NULL				primary role in			His78		statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_6778_s_12	14672943	His78 appears to play the primary role in the specific binding of heme to the NTD, acting analogously to the "`proximal histidine"` ligand of globins, while His123 appears to act as the "`distal"` heme ligand.	transcription
66535	3	335702	7	NULL	NULL	0	NULL				act analogously to			His78 		globins	GP	ligand of	proximal histidine		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_6778_s_12	14672943	His78 appears to play the primary role in the specific binding of heme to the NTD, acting analogously to the "`proximal histidine"` ligand of globins, while His123 appears to act as the "`distal"` heme ligand.	transcription
66536	4	335702	7	NULL	NULL	0	NULL				act as			His123		heme ligand	GP		distal		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_6778_s_12	14672943	His78 appears to play the primary role in the specific binding of heme to the NTD, acting analogously to the "`proximal histidine"` ligand of globins, while His123 appears to act as the "`distal"` heme ligand.	transcription
56726	1	335703	5	NULL	NULL	0	NULL	globin genes		transcriptional activation of	results in					globin chains		synthesis of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_51_4_558_s_28	9106619	The synthesis of globin chains primarily results from transcriptional activation of the globin genes ( 16), and the enhanced heme production is ensured by activation of the enzymes responsible for its biosynthesis.	transcription
56727	2	335703	5	NULL	NULL	0	NULL	statement 1			enhances					heme		production of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_51_4_558_s_28	9106619	The synthesis of globin chains primarily results from transcriptional activation of the globin genes ( 16), and the enhanced heme production is ensured by activation of the enzymes responsible for its biosynthesis.	transcription
66537	1	335703	7	NULL	NULL	0	NULL	globin chains	GP	synthesis of	result from					globin genes	GP	transcriptional activation of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_51_4_558_s_28	9106619	The synthesis of globin chains primarily results from transcriptional activation of the globin genes ( 16), and the enhanced heme production is ensured by activation of the enzymes responsible for its biosynthesis.	transcription
56728	1	335704	5	NULL	NULL	0	NULL	beta-globin chains		expressed	bind					heme					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_43_26677_s_147	8900144	Expressed beta-globin chains bound heme and spectrophotometric properties were similar to that of authentic beta-globin from human red blood cells.	transcription
66538	1	335704	7	NULL	NULL	0	NULL	beta-globin chains	GP	expressed	bind					heme	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_43_26677_s_147	8900144	Expressed beta-globin chains bound heme and spectrophotometric properties were similar to that of authentic beta-globin from human red blood cells.	transcription
56729	1	335705	5	NULL	NULL	0	NULL	beta-globin gene		regulation of;;expression of	is dependent on					heme					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_4	14660636	To investigate the involvement of Bach1 in the heme-dependent regulation of the expression of the beta-globin gene, mouse erythroleukemia (MEL) cells were cultured with succinylacetone (SA), a specific inhibitor of heme biosynthesis, and the level of beta-globin mRNA was examined.	transcription
56730	2	335705	5	NULL	NULL	0	NULL	Bach1			is involved in		potentially			statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_4	14660636	To investigate the involvement of Bach1 in the heme-dependent regulation of the expression of the beta-globin gene, mouse erythroleukemia (MEL) cells were cultured with succinylacetone (SA), a specific inhibitor of heme biosynthesis, and the level of beta-globin mRNA was examined.	transcription
66539	1	335705	7	NULL	NULL	0	NULL	SA	Chemical		is an inhibitor of					heme biosynthesis	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_4	14660636	To investigate the involvement of Bach1 in the heme-dependent regulation of the expression of the beta-globin gene, mouse erythroleukemia (MEL) cells were cultured with succinylacetone (SA), a specific inhibitor of heme biosynthesis, and the level of beta-globin mRNA was examined.	transcription
66540	2	335705	7	NULL	NULL	0	NULL	SA	Chemical		is					succinylacetone 	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_4	14660636	To investigate the involvement of Bach1 in the heme-dependent regulation of the expression of the beta-globin gene, mouse erythroleukemia (MEL) cells were cultured with succinylacetone (SA), a specific inhibitor of heme biosynthesis, and the level of beta-globin mRNA was examined.	transcription
56731	1	335706	5	NULL	NULL	0	NULL	Bach1			regulates		potentially			beta-globin gene		expression of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_40	14660636	To clarify whether Bach1 regulates beta-globin gene expression, we examined heme-dependent expression of the beta-globin gene in human erythroleukemia K562 and MEL cells and the regulation of the interaction of Bach1 with the LCR by heme.	transcription
56732	2	335706	5	NULL	NULL	0	NULL	Bach1			interacts with					LCR					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_40	14660636	To clarify whether Bach1 regulates beta-globin gene expression, we examined heme-dependent expression of the beta-globin gene in human erythroleukemia K562 and MEL cells and the regulation of the interaction of Bach1 with the LCR by heme.	transcription
66541	1	335706	7	NULL	NULL	0	NULL	 beta-globin gene	GP	expression of	depends on					heme	Chemical				NULL	human erythroleukemia K562 cells	0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_40	14660636	To clarify whether Bach1 regulates beta-globin gene expression, we examined heme-dependent expression of the beta-globin gene in human erythroleukemia K562 and MEL cells and the regulation of the interaction of Bach1 with the LCR by heme.	transcription
66542	2	335706	7	NULL	NULL	0	NULL	beta-globin gene	GP	expression of	depends on					heme	Chemical				NULL	MEL cells	0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_40	14660636	To clarify whether Bach1 regulates beta-globin gene expression, we examined heme-dependent expression of the beta-globin gene in human erythroleukemia K562 and MEL cells and the regulation of the interaction of Bach1 with the LCR by heme.	transcription
66543	3	335706	7	NULL	NULL	0	NULL	Bach1	GP		interacts with					LCR	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_40	14660636	To clarify whether Bach1 regulates beta-globin gene expression, we examined heme-dependent expression of the beta-globin gene in human erythroleukemia K562 and MEL cells and the regulation of the interaction of Bach1 with the LCR by heme.	transcription
66544	4	335706	7	NULL	NULL	0	NULL	heme	Chemical		regulates					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_40	14660636	To clarify whether Bach1 regulates beta-globin gene expression, we examined heme-dependent expression of the beta-globin gene in human erythroleukemia K562 and MEL cells and the regulation of the interaction of Bach1 with the LCR by heme.	transcription
56733	1	335707	5	NULL	NULL	0	NULL	heme		inhibition of;;biosynthesis of	decreases					beta-globin		expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_101	14660636	The decreased beta-globin expression by the inhibition of heme biosynthesis was reversed by culture with 50 muM hemin, suggesting that the expression of beta-globin mRNA in MEL cells is controlled by heme in both uninduced and induced cells.	transcription
56734	2	335707	5	NULL	NULL	0	NULL	hemin			reverses					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_101	14660636	The decreased beta-globin expression by the inhibition of heme biosynthesis was reversed by culture with 50 muM hemin, suggesting that the expression of beta-globin mRNA in MEL cells is controlled by heme in both uninduced and induced cells.	transcription
56735	3	335707	5	NULL	NULL	0	NULL	beta-globin mRNA			is expressed in					MEL cells					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_101	14660636	The decreased beta-globin expression by the inhibition of heme biosynthesis was reversed by culture with 50 muM hemin, suggesting that the expression of beta-globin mRNA in MEL cells is controlled by heme in both uninduced and induced cells.	transcription
56736	4	335707	5	NULL	NULL	0	NULL	heme			controls					statement 3					NULL	uninduced cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_101	14660636	The decreased beta-globin expression by the inhibition of heme biosynthesis was reversed by culture with 50 muM hemin, suggesting that the expression of beta-globin mRNA in MEL cells is controlled by heme in both uninduced and induced cells.	transcription
56737	5	335707	5	NULL	NULL	0	NULL	heme			controls					statement 3					NULL	induced cells	0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_101	14660636	The decreased beta-globin expression by the inhibition of heme biosynthesis was reversed by culture with 50 muM hemin, suggesting that the expression of beta-globin mRNA in MEL cells is controlled by heme in both uninduced and induced cells.	transcription
66545	1	335707	7	NULL	NULL	0	NULL	beta-globin mRNA	GP	expression of	is controlled by					heme	Chemical				NULL	induced MEL cells	0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_101	14660636	The decreased beta-globin expression by the inhibition of heme biosynthesis was reversed by culture with 50 muM hemin, suggesting that the expression of beta-globin mRNA in MEL cells is controlled by heme in both uninduced and induced cells.	transcription
66546	2	335707	7	NULL	NULL	NULL	NULL	beta-globin mRNA	GP	expression of	is controlled by					heme	Chemical				NULL	uninduced MEL cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_101	14660636	The decreased beta-globin expression by the inhibition of heme biosynthesis was reversed by culture with 50 muM hemin, suggesting that the expression of beta-globin mRNA in MEL cells is controlled by heme in both uninduced and induced cells.	transcription
66547	3	335707	7	NULL	NULL	0	NULL	heme biosynthesis	Process	inhibition of	decrease					beta-globin	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_101	14660636	The decreased beta-globin expression by the inhibition of heme biosynthesis was reversed by culture with 50 muM hemin, suggesting that the expression of beta-globin mRNA in MEL cells is controlled by heme in both uninduced and induced cells.	transcription
66548	4	335707	7	NULL	NULL	0	NULL	heme	Chemical		reverse					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_101	14660636	The decreased beta-globin expression by the inhibition of heme biosynthesis was reversed by culture with 50 muM hemin, suggesting that the expression of beta-globin mRNA in MEL cells is controlled by heme in both uninduced and induced cells.	transcription
56738	1	335708	5	NULL	NULL	0	NULL	heme			not incorporated into					beta-globin					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_43_26677_s_138	8900144	From these results they suggested that heme was not incorporated into beta-globin and that interaction between alpha-and beta-globin chains may affect correct folding of the two globin polypeptides in  E. coli ( 4).	transcription
56739	2	335708	5	NULL	NULL	0	NULL	alpha-globin chains			interacts with					beta-globin chains					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_43_26677_s_138	8900144	From these results they suggested that heme was not incorporated into beta-globin and that interaction between alpha-and beta-globin chains may affect correct folding of the two globin polypeptides in  E. coli ( 4).	transcription
56740	3	335708	5	NULL	NULL	0	NULL	statement 2			affects		may			globin polypeptides		correct folding of			NULL	E. coli	0	NULL	NULL	NULL	gw60_jbiolchem_271_43_26677_s_138	8900144	From these results they suggested that heme was not incorporated into beta-globin and that interaction between alpha-and beta-globin chains may affect correct folding of the two globin polypeptides in  E. coli ( 4).	transcription
66549	1	335708	7	NULL	NULL	0	NULL	alpha-globin chain	GP		interacts with					beta-globin chain	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_43_26677_s_138	8900144	From these results they suggested that heme was not incorporated into beta-globin and that interaction between alpha-and beta-globin chains may affect correct folding of the two globin polypeptides in  E. coli ( 4).	transcription
66550	2	335708	7	NULL	NULL	0	NULL	statement 1	Process		affect		may			two globin polypeptides	GP	correct folding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_43_26677_s_138	8900144	From these results they suggested that heme was not incorporated into beta-globin and that interaction between alpha-and beta-globin chains may affect correct folding of the two globin polypeptides in  E. coli ( 4).	transcription
56741	1	335709	5	NULL	NULL	0	NULL	heme group			is a constituent of		intimate			globin molecule					NULL		0	NULL	NULL	NULL	gw70_pnas_102_48_17320_s_133	16301540	The heme group is an intimate constituent of the globin molecule, and mutations of amino acids that line the heme-binding site in myoglobin affect protein folding and stability ( ).	transcription
66551	1	335709	7	NULL	NULL	0	NULL	heme group	GP		intimate constituent of					globin molecule	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_102_48_17320_s_133	16301540	The heme group is an intimate constituent of the globin molecule, and mutations of amino acids that line the heme-binding site in myoglobin affect protein folding and stability ( ).	transcription
66552	2	335709	7	NULL	NULL	NULL	NULL	myoglobin	GP	mutations in	affect			aminoacid lining heme-binding site		protein folding	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_48_17320_s_133	16301540	The heme group is an intimate constituent of the globin molecule, and mutations of amino acids that line the heme-binding site in myoglobin affect protein folding and stability ( ).	transcription
66553	3	335709	7	NULL	NULL	NULL	NULL	myoglobin	GP	mutations in	affect			aminoacid lining heme-binding site		protein stability	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_102_48_17320_s_133	16301540	The heme group is an intimate constituent of the globin molecule, and mutations of amino acids that line the heme-binding site in myoglobin affect protein folding and stability ( ).	transcription
56742	1	335710	5	NULL	NULL	0	NULL	heme			is synthesized during					erythroid		differentiation of			NULL		0	NULL	NULL	NULL	gw70_pnas_101_6_1461_s_182	14747657	Because heme is synthesized at high levels during erythroid differentiation, we investigated whether heme induces displacement of Bach1 from the beta-globin LCR.	transcription
56743	2	335710	5	NULL	NULL	0	NULL	Bach1			displaced from					beta-globin				LCR	NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_6_1461_s_182	14747657	Because heme is synthesized at high levels during erythroid differentiation, we investigated whether heme induces displacement of Bach1 from the beta-globin LCR.	transcription
56744	3	335710	5	NULL	NULL	0	NULL	heme			induces		potentially			statement 2					NULL		0	NULL	NULL	NULL	gw70_pnas_101_6_1461_s_182	14747657	Because heme is synthesized at high levels during erythroid differentiation, we investigated whether heme induces displacement of Bach1 from the beta-globin LCR.	transcription
66554	1	335710	7	NULL	NULL	0	NULL	heme	Chemical	high levels of	synthesized during					erythroid differentiation	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_101_6_1461_s_182	14747657	Because heme is synthesized at high levels during erythroid differentiation, we investigated whether heme induces displacement of Bach1 from the beta-globin LCR.	transcription
56759	1	335711	5	NULL	NULL	0	NULL	globin		proximal side of	contains			heme pocket					side chains at Leu89(F4)		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_12_9093_s_4	11084036	Globin side chains at the Leu89(F4), His97(FG3), Ile99(FG5), and Leu104(G5) positions on the proximal side of the heme pocket strongly influence heme affinity.	transcription
56760	2	335711	5	NULL	NULL	0	NULL	globin		proximal side of	contains			heme pocket					side chains at His97(FG3)		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_12_9093_s_4	11084036	Globin side chains at the Leu89(F4), His97(FG3), Ile99(FG5), and Leu104(G5) positions on the proximal side of the heme pocket strongly influence heme affinity.	transcription
56761	3	335711	5	NULL	NULL	0	NULL	globin		proximal side of	contains			heme pocket					side chains at Ile99(FG5)		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_12_9093_s_4	11084036	Globin side chains at the Leu89(F4), His97(FG3), Ile99(FG5), and Leu104(G5) positions on the proximal side of the heme pocket strongly influence heme affinity.	transcription
56763	4	335711	5	NULL	NULL	0	NULL	globin		proximal side of	contains			heme pocket					side chains at Leu104(G5)		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_12_9093_s_4	11084036	Globin side chains at the Leu89(F4), His97(FG3), Ile99(FG5), and Leu104(G5) positions on the proximal side of the heme pocket strongly influence heme affinity.	transcription
56764	5	335711	5	NULL	NULL	0	NULL	statement 1			influences		strongly			heme		affinity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_12_9093_s_4	11084036	Globin side chains at the Leu89(F4), His97(FG3), Ile99(FG5), and Leu104(G5) positions on the proximal side of the heme pocket strongly influence heme affinity.	transcription
56765	6	335711	5	NULL	NULL	0	NULL	statement 2			influences		strongly			heme		affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_12_9093_s_4	11084036	Globin side chains at the Leu89(F4), His97(FG3), Ile99(FG5), and Leu104(G5) positions on the proximal side of the heme pocket strongly influence heme affinity.	transcription
56766	7	335711	5	NULL	NULL	0	NULL	statement 3			influences		strongly			heme		affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_12_9093_s_4	11084036	Globin side chains at the Leu89(F4), His97(FG3), Ile99(FG5), and Leu104(G5) positions on the proximal side of the heme pocket strongly influence heme affinity.	transcription
56767	8	335711	5	NULL	NULL	0	NULL	statement 4			influences		strongly			heme		affinity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_12_9093_s_4	11084036	Globin side chains at the Leu89(F4), His97(FG3), Ile99(FG5), and Leu104(G5) positions on the proximal side of the heme pocket strongly influence heme affinity.	transcription
66555	1	335711	7	NULL	NULL	NULL	NULL	Globin	GP		influence		strongly	 side chain Leu89(F4) positions on the proximal side of the heme pocket		heme affinity	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_12_9093_s_4	11084036	Globin side chains at the Leu89(F4), His97(FG3), Ile99(FG5), and Leu104(G5) positions on the proximal side of the heme pocket strongly influence heme affinity.	transcription
66556	2	335711	7	NULL	NULL	NULL	NULL	Globin	GP		influence		strongly	side chain His97(FG3) positions on the proximal side of the heme pocket		heme affinity	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_12_9093_s_4	11084036	Globin side chains at the Leu89(F4), His97(FG3), Ile99(FG5), and Leu104(G5) positions on the proximal side of the heme pocket strongly influence heme affinity.	transcription
66557	3	335711	7	NULL	NULL	NULL	NULL	Globin	GP		influence		strongly	side chain Ile99(FG5) positions on the proximal side of the heme pocket		heme affinity	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_12_9093_s_4	11084036	Globin side chains at the Leu89(F4), His97(FG3), Ile99(FG5), and Leu104(G5) positions on the proximal side of the heme pocket strongly influence heme affinity.	transcription
66558	4	335711	7	NULL	NULL	0	NULL	Globin	GP		influence		strongly	side chain Leu104(G5) positions on the proximal side of the heme pocket		heme affinity	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_12_9093_s_4	11084036	Globin side chains at the Leu89(F4), His97(FG3), Ile99(FG5), and Leu104(G5) positions on the proximal side of the heme pocket strongly influence heme affinity.	transcription
56745	1	335712	5	NULL	NULL	0	NULL	HRI			is					heme- regulated inhibitor					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_206_s_12	11036079	The  heme- regulated  inhibitor (HRI)1 of protein synthesis is a protein-serine kinase which coordinates the synthesis of globin chains with the availability of heme in reticulocytes (reviewed in Refs.	transcription
56746	2	335712	5	NULL	NULL	0	NULL	(HRI)1			is a type of					protein-serine kinase					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_206_s_12	11036079	The  heme- regulated  inhibitor (HRI)1 of protein synthesis is a protein-serine kinase which coordinates the synthesis of globin chains with the availability of heme in reticulocytes (reviewed in Refs.	transcription
56747	3	335712	5	NULL	NULL	0	NULL	globin chains		synthesis of	coordinates with					heme		availability of			NULL	reticulocytes	0	NULL	NULL	NULL	gw60_jbiolchem_276_1_206_s_12	11036079	The  heme- regulated  inhibitor (HRI)1 of protein synthesis is a protein-serine kinase which coordinates the synthesis of globin chains with the availability of heme in reticulocytes (reviewed in Refs.	transcription
56748	4	335712	5	NULL	NULL	0	NULL	(HRI)1			is required for					statement 3					NULL	reticulocytes	0	NULL	NULL	NULL	gw60_jbiolchem_276_1_206_s_12	11036079	The  heme- regulated  inhibitor (HRI)1 of protein synthesis is a protein-serine kinase which coordinates the synthesis of globin chains with the availability of heme in reticulocytes (reviewed in Refs.	transcription
66559	1	335712	7	NULL	NULL	0	NULL	HRI	GP		is a type of					protein-serine kinase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_206_s_12	11036079	The  heme- regulated  inhibitor (HRI)1 of protein synthesis is a protein-serine kinase which coordinates the synthesis of globin chains with the availability of heme in reticulocytes (reviewed in Refs.	transcription
66560	2	335712	7	NULL	NULL	0	NULL	HRI	GP		coordinate					globin chains	GP	synthesis of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_206_s_12	11036079	The  heme- regulated  inhibitor (HRI)1 of protein synthesis is a protein-serine kinase which coordinates the synthesis of globin chains with the availability of heme in reticulocytes (reviewed in Refs.	transcription
66561	3	335712	7	NULL	NULL	0	NULL	statement 1	Process		depends on					heme	Chemical	availability of			NULL	reticulocytes	0	NULL	NULL	NULL	gw60_jbiolchem_276_1_206_s_12	11036079	The  heme- regulated  inhibitor (HRI)1 of protein synthesis is a protein-serine kinase which coordinates the synthesis of globin chains with the availability of heme in reticulocytes (reviewed in Refs.	transcription
66562	4	335712	7	NULL	NULL	0	NULL	HRI	GP		is					heme- regulated inhibitor	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_206_s_12	11036079	The  heme- regulated  inhibitor (HRI)1 of protein synthesis is a protein-serine kinase which coordinates the synthesis of globin chains with the availability of heme in reticulocytes (reviewed in Refs.	transcription
66563	1	335713	7	NULL	NULL	0	NULL	heme binding module	GP		regulates					globin family	GP		heme proximal structure in		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_17_12438_s_20	10777528	In our previous paper ( 13), we have proposed the heme binding module, a protein continuous segment regulating the heme proximal structure in the globin family.	transcription
56749	1	335714	5	NULL	NULL	0	NULL	globin			has affinity for		high			heme					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_51_47937_s_190	11602592	No heme exchange reaction was demonstrated between ferrous and ferric Hb because of the high affinity of globin for the heme ( 19); such an exchange would involve a concomitant heme dissociation from both types of subunit.	transcription
66564	1	335714	7	NULL	NULL	0	NULL	globin	GP		high affinity for					heme	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_51_47937_s_190	11602592	No heme exchange reaction was demonstrated between ferrous and ferric Hb because of the high affinity of globin for the heme ( 19); such an exchange would involve a concomitant heme dissociation from both types of subunit.	transcription
56750	1	335715	5	NULL	NULL	0	NULL	heme			bind					cytochromes					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_51_32605_s_173	8955088	The loose association of heme with these proteins is quite different from the situation observed for heme binding to cytochromes, globin, or other heme-binding proteins (see  e.g. 38), where a stable interaction is needed to ensure proper biochemical function.	transcription
56751	2	335715	5	NULL	NULL	0	NULL	heme			bind					globin					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_51_32605_s_173	8955088	The loose association of heme with these proteins is quite different from the situation observed for heme binding to cytochromes, globin, or other heme-binding proteins (see  e.g. 38), where a stable interaction is needed to ensure proper biochemical function.	transcription
66565	1	335715	7	NULL	NULL	0	NULL	heme	Chemical		bind					cytochromes	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_51_32605_s_173	8955088	The loose association of heme with these proteins is quite different from the situation observed for heme binding to cytochromes, globin, or other heme-binding proteins (see  e.g. 38), where a stable interaction is needed to ensure proper biochemical function.	transcription
66566	2	335715	7	NULL	NULL	0	NULL	heme	Chemical		bind					globin	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_51_32605_s_173	8955088	The loose association of heme with these proteins is quite different from the situation observed for heme binding to cytochromes, globin, or other heme-binding proteins (see  e.g. 38), where a stable interaction is needed to ensure proper biochemical function.	transcription
66567	3	335715	7	NULL	NULL	0	NULL	statement 1	Process	stable interaction of	is required for					biochemical function	Process	proper			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_51_32605_s_173	8955088	The loose association of heme with these proteins is quite different from the situation observed for heme binding to cytochromes, globin, or other heme-binding proteins (see  e.g. 38), where a stable interaction is needed to ensure proper biochemical function.	transcription
66568	4	335715	7	NULL	NULL	0	NULL	statement 2	Process	stable interaction of	is required for					biochemical function	Process	proper			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_51_32605_s_173	8955088	The loose association of heme with these proteins is quite different from the situation observed for heme binding to cytochromes, globin, or other heme-binding proteins (see  e.g. 38), where a stable interaction is needed to ensure proper biochemical function.	transcription
56752	1	335716	5	NULL	NULL	0	NULL	globin			bind			chain a		heme					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_47_29999_s_181	8939946	The conclusion that the stoichiometry is ( abcd)2L implies that the calculation of heme content hinges on whether the linkers bind any heme because the globin chains  a,  b,  c, and  d each bind heme.	transcription
56753	2	335716	5	NULL	NULL	0	NULL	globin			bind			chain b		heme					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_47_29999_s_181	8939946	The conclusion that the stoichiometry is ( abcd)2L implies that the calculation of heme content hinges on whether the linkers bind any heme because the globin chains  a,  b,  c, and  d each bind heme.	transcription
56754	3	335716	5	NULL	NULL	0	NULL	globin			bind			chain c		heme					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_47_29999_s_181	8939946	The conclusion that the stoichiometry is ( abcd)2L implies that the calculation of heme content hinges on whether the linkers bind any heme because the globin chains  a,  b,  c, and  d each bind heme.	transcription
56755	4	335716	5	NULL	NULL	0	NULL	globin			bind			chain d		heme					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_47_29999_s_181	8939946	The conclusion that the stoichiometry is ( abcd)2L implies that the calculation of heme content hinges on whether the linkers bind any heme because the globin chains  a,  b,  c, and  d each bind heme.	transcription
66569	1	335716	7	NULL	NULL	NULL	NULL	 globin 	GP		bind			chain a		heme	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_47_29999_s_181	8939946	The conclusion that the stoichiometry is ( abcd)2L implies that the calculation of heme content hinges on whether the linkers bind any heme because the globin chains  a,  b,  c, and  d each bind heme.	transcription
66570	2	335716	7	NULL	NULL	NULL	NULL	globin	GP		bind			chain b		heme	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_47_29999_s_181	8939946	The conclusion that the stoichiometry is ( abcd)2L implies that the calculation of heme content hinges on whether the linkers bind any heme because the globin chains  a,  b,  c, and  d each bind heme.	transcription
66571	3	335716	7	NULL	NULL	0	NULL	globin	GP		bind			chain c		heme	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_47_29999_s_181	8939946	The conclusion that the stoichiometry is ( abcd)2L implies that the calculation of heme content hinges on whether the linkers bind any heme because the globin chains  a,  b,  c, and  d each bind heme.	transcription
56756	1	335717	5	NULL	NULL	0	NULL	globin gene		stimulation of;;expression of	is dependent on					heme					NULL	erythroid precursor cells	0	NULL	NULL	NULL	gw70_biochimbiophysacta_1619_2_113_s_141	12527106	Increased NF-E2 binding probably accounts for heme-dependent stimulation of globin  gene expression in erythroid precursor cells [ 71 and  82].	transcription
56757	2	335717	5	NULL	NULL	0	NULL	NF-E2		increased binding of	accounts for		probably			statement 1					NULL	erythroid precursor cells	NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1619_2_113_s_141	12527106	Increased NF-E2 binding probably accounts for heme-dependent stimulation of globin  gene expression in erythroid precursor cells [ 71 and  82].	transcription
66582	1	335717	7	NULL	NULL	0	NULL	globin gene	GP	stimulation of;;expression of	depends on					heme	Chemical				NULL	erythroid precursor cells	0	NULL	NULL	NULL	gw70_biochimbiophysacta_1619_2_113_s_141	12527106	Increased NF-E2 binding probably accounts for heme-dependent stimulation of globin  gene expression in erythroid precursor cells [ 71 and  82].	transcription
66585	2	335717	7	NULL	NULL	NULL	NULL	statement 1	Process		increase					NF-E2	GP	binding of			NULL		NULL	NULL	NULL	NULL	gw70_biochimbiophysacta_1619_2_113_s_141	12527106	Increased NF-E2 binding probably accounts for heme-dependent stimulation of globin  gene expression in erythroid precursor cells [ 71 and  82].	transcription
66586	1	335718	7	NULL	NULL	0	NULL	heme	Chemical		bind					globin	GP				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_305_4_840_s_284	12767907	M.S. Hargrove, D. Barrick and J.S. Olson, The association rate constant for heme  binding to globin is independent of protein structure.	transcription
66587	2	335718	7	NULL	NULL	0	NULL	statement 1	Process		is independent of					protein structure					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_305_4_840_s_284	12767907	M.S. Hargrove, D. Barrick and J.S. Olson, The association rate constant for heme  binding to globin is independent of protein structure.	transcription
56768	1	335719	5	NULL	NULL	0	NULL	Transthyretin			interacts with					globin					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_311_2_344_s_354	14592420	R. Martone and J. Herbert, Transthyretin interacts with globin to form protein complexes  with heme dependent solubility.	transcription
66588	1	335719	7	NULL	NULL	0	NULL	Transthyretin	GP		interacts with					globin	GP				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_311_2_344_s_354	14592420	R. Martone and J. Herbert, Transthyretin interacts with globin to form protein complexes  with heme dependent solubility.	transcription
66589	2	335719	7	NULL	NULL	0	NULL	statement 1	Process		form					protein complexes	GP				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_311_2_344_s_354	14592420	R. Martone and J. Herbert, Transthyretin interacts with globin to form protein complexes  with heme dependent solubility.	transcription
66590	3	335719	7	NULL	NULL	0	NULL	solubility	Process		depends on					heme 	Chemical				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_311_2_344_s_354	14592420	R. Martone and J. Herbert, Transthyretin interacts with globin to form protein complexes  with heme dependent solubility.	transcription
66591	4	335719	7	NULL	NULL	0	NULL	statement 2	Process		occur with					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_311_2_344_s_354	14592420	R. Martone and J. Herbert, Transthyretin interacts with globin to form protein complexes  with heme dependent solubility.	transcription
56769	1	335720	5	NULL	NULL	0	NULL	heme			regulates		positively			beta-globin		expression of		locus control region	NULL	erythroid cells	0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_1	14660636	Heme positively regulates the expression of beta-globin at the locus control region via the transcriptional factor Bach1 in erythroid cells.	transcription
56770	2	335720	5	NULL	NULL	0	NULL	statement 1			via					Bach1					NULL	erythroid cells	0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_1	14660636	Heme positively regulates the expression of beta-globin at the locus control region via the transcriptional factor Bach1 in erythroid cells.	transcription
56771	3	335720	5	NULL	NULL	0	NULL	Bach1			is a type of					transcription factor					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_1	14660636	Heme positively regulates the expression of beta-globin at the locus control region via the transcriptional factor Bach1 in erythroid cells.	transcription
66592	1	335720	7	NULL	NULL	0	NULL	Heme	Chemical		regulates		positively			beta-globin	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_1	14660636	Heme positively regulates the expression of beta-globin at the locus control region via the transcriptional factor Bach1 in erythroid cells.	transcription
66593	2	335720	7	NULL	NULL	NULL	NULL	statement 1	Process		occur at					locus control region	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_1	14660636	Heme positively regulates the expression of beta-globin at the locus control region via the transcriptional factor Bach1 in erythroid cells.	transcription
66594	3	335720	7	NULL	NULL	0	NULL	statement 1	Process		via					Bach1	GP				NULL	erythroid cells	0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_1	14660636	Heme positively regulates the expression of beta-globin at the locus control region via the transcriptional factor Bach1 in erythroid cells.	transcription
66595	4	335720	7	NULL	NULL	0	NULL	Bach1	GP		is a type of					transcription factor	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_1	14660636	Heme positively regulates the expression of beta-globin at the locus control region via the transcriptional factor Bach1 in erythroid cells.	transcription
56772	1	335721	5	NULL	NULL	0	NULL	Bach1			interacts with									MARE in LCR	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_14	14660636	We propose that heme positively regulates the beta-globin gene expression by blocking the interaction of Bach1 with the MARE in the LCR.	transcription
56773	2	335721	5	NULL	NULL	0	NULL	heme			regulates		positively			beta-globin gene		expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_14	14660636	We propose that heme positively regulates the beta-globin gene expression by blocking the interaction of Bach1 with the MARE in the LCR.	transcription
56774	3	335721	5	NULL	NULL	0	NULL	heme			blocks					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_14	14660636	We propose that heme positively regulates the beta-globin gene expression by blocking the interaction of Bach1 with the MARE in the LCR.	transcription
56775	4	335721	5	NULL	NULL	0	NULL	statement 3			leads to					statement 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_14	14660636	We propose that heme positively regulates the beta-globin gene expression by blocking the interaction of Bach1 with the MARE in the LCR.	transcription
66625	1	335721	7	NULL	NULL	0	NULL	heme	Chemical		regulates		positively			beta-globin gene	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_14	14660636	We propose that heme positively regulates the beta-globin gene expression by blocking the interaction of Bach1 with the MARE in the LCR.	transcription
66626	2	335721	7	NULL	NULL	NULL	NULL	Bach1	GP		interacts with									MARE	NULL	LCR	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_14	14660636	We propose that heme positively regulates the beta-globin gene expression by blocking the interaction of Bach1 with the MARE in the LCR.	transcription
66662	3	335721	7	NULL	NULL	0	NULL	statement 1	Process		occur by					statement 2	Process	blocking 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_14	14660636	We propose that heme positively regulates the beta-globin gene expression by blocking the interaction of Bach1 with the MARE in the LCR.	transcription
56776	1	335722	5	NULL	NULL	0	NULL	Bach1			interacts with									LCR	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_41	14660636	Here we demonstrated that heme positively regulates the beta-globin gene expression by disrupting the interaction of Bach1 with the LCR.	transcription
56777	2	335722	5	NULL	NULL	0	NULL	heme			disrupts					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_41	14660636	Here we demonstrated that heme positively regulates the beta-globin gene expression by disrupting the interaction of Bach1 with the LCR.	transcription
56778	3	335722	5	NULL	NULL	0	NULL	heme			regulates		positively			beta-globin gene		expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_41	14660636	Here we demonstrated that heme positively regulates the beta-globin gene expression by disrupting the interaction of Bach1 with the LCR.	transcription
56779	4	335722	5	NULL	NULL	0	NULL	statement 2			leads to					statement 3					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_41	14660636	Here we demonstrated that heme positively regulates the beta-globin gene expression by disrupting the interaction of Bach1 with the LCR.	transcription
66663	1	335722	7	NULL	NULL	0	NULL	heme	Chemical		regulates		positively			beta-globin gene	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_41	14660636	Here we demonstrated that heme positively regulates the beta-globin gene expression by disrupting the interaction of Bach1 with the LCR.	transcription
66664	2	335722	7	NULL	NULL	0	NULL	Bach1	GP		interacts with					LCR	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_41	14660636	Here we demonstrated that heme positively regulates the beta-globin gene expression by disrupting the interaction of Bach1 with the LCR.	transcription
66667	3	335722	7	NULL	NULL	0	NULL	statement 1	Process		occur by					statement 2	Process	disrupting			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_41	14660636	Here we demonstrated that heme positively regulates the beta-globin gene expression by disrupting the interaction of Bach1 with the LCR.	transcription
56800	1	335723	5	NULL	NULL	0	NULL	heme			bind		covalently			apo-globin			His-120		NULL		0	NULL	NULL	NULL	gw70_pnas_101_17_6675_s_166	15096613	Mutagenesis experiments coupled with our 3D homology model of  ApPgb indicate that heme is covalently bound to the apo-globin by means of His-120.	transcription
79028	1	335723	6	NULL	NULL	0	NULL	heme	GP		bind			His-120		apo-globin	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_17_6675_s_166	15096613	Mutagenesis experiments coupled with our 3D homology model of  ApPgb indicate that heme is covalently bound to the apo-globin by means of His-120.	transcription
56801	1	335724	5	NULL	NULL	0	NULL	Bach1			departs from		selectively			beta-globin				MAREs	NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_6_1461_s_189	14747657	Thus, heme induced the selective departure of Bach1 from the beta-globin MAREs without affecting the binding of MafK.	transcription
56802	2	335724	5	NULL	NULL	0	NULL	heme			induce					statement 1					NULL		0	NULL	NULL	NULL	gw70_pnas_101_6_1461_s_189	14747657	Thus, heme induced the selective departure of Bach1 from the beta-globin MAREs without affecting the binding of MafK.	transcription
56803	3	335724	5	NULL	NULL	0	NULL	statement 2			does not affect					MafK		binding of			NULL		0	NULL	NULL	NULL	gw70_pnas_101_6_1461_s_189	14747657	Thus, heme induced the selective departure of Bach1 from the beta-globin MAREs without affecting the binding of MafK.	transcription
79029	1	335724	6	NULL	NULL	0	NULL	Bach1	GP		bind					beta-globin	GP			MARE	NULL		0	NULL	NULL	NULL	gw70_pnas_101_6_1461_s_189	14747657	Thus, heme induced the selective departure of Bach1 from the beta-globin MAREs without affecting the binding of MafK.	transcription
56804	1	335727	5	NULL	NULL	0	NULL	heme			bind					globin					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_12_9093_s_14	11084036	Heme binding causes the globin to form a more compact structure with an approximately 20% increase in helicity ( 1).	transcription
56805	1	335728	5	NULL	NULL	0	NULL	heme			bind					alpha-globin		rabbit			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_52_32715_s_38	9407040	Binding of heme to rabbit alpha-globin begins when the emerging polypeptide achieves a length of 86 residues ( 19).	transcription
79030	1	335728	6	NULL	NULL	0	NULL	heme	GP		bind					alpha-globin	GP	rabbit			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_52_32715_s_38	9407040	Binding of heme to rabbit alpha-globin begins when the emerging polypeptide achieves a length of 86 residues ( 19).	transcription
56806	1	335729	5	NULL	NULL	0	NULL	heme		binding of	induce					globin molecule		conformational shift of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_37_28659_s_179	10896678	This observation could mean that the binding of heme induced a conformational shift in the globin molecule leading to exposure of susceptible peptide bonds.	transcription
56807	2	335729	5	NULL	NULL	0	NULL	statement 1			exposes					peptide bonds		susceptible			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_37_28659_s_179	10896678	This observation could mean that the binding of heme induced a conformational shift in the globin molecule leading to exposure of susceptible peptide bonds.	transcription
56808	1	335730	5	NULL	NULL	0	NULL	heme			bind					globin					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_23_13785_s_11	7775434	This suggested that binding of heme to  globin and binding of     dimers to each other are yet another  example of linked functions.	transcription
56809	1	335732	5	NULL	NULL	0	NULL	globin gene			is activated by					heme					NULL		0	NULL	NULL	NULL	abs-batch0600-0619_antioxid-redox-signal_8_1-2_16487039_s_9	16487039	Our results suggest that globin  gene activation by heme appears to be independent of the putative HRMs  in the p45 subunit of the NF-E2 transcription factor.	transcription
56810	2	335732	5	NULL	NULL	0	NULL	NF-E2			is a type of					transcription factor					NULL		0	NULL	NULL	NULL	abs-batch0600-0619_antioxid-redox-signal_8_1-2_16487039_s_9	16487039	Our results suggest that globin  gene activation by heme appears to be independent of the putative HRMs  in the p45 subunit of the NF-E2 transcription factor.	transcription
56811	3	335732	5	NULL	NULL	0	NULL	NF-E2			contains			p45 subunit				putative	HRMs		NULL		0	NULL	NULL	NULL	abs-batch0600-0619_antioxid-redox-signal_8_1-2_16487039_s_9	16487039	Our results suggest that globin  gene activation by heme appears to be independent of the putative HRMs  in the p45 subunit of the NF-E2 transcription factor.	transcription
56812	4	335732	5	NULL	NULL	0	NULL	statement 1			is independent of					statement 3					NULL		0	NULL	NULL	NULL	abs-batch0600-0619_antioxid-redox-signal_8_1-2_16487039_s_9	16487039	Our results suggest that globin  gene activation by heme appears to be independent of the putative HRMs  in the p45 subunit of the NF-E2 transcription factor.	transcription
79031	1	335732	6	NULL	NULL	0	NULL	heme	GP		activates					globin gene	GP				NULL		0	NULL	NULL	NULL	abs-batch0600-0619_antioxid-redox-signal_8_1-2_16487039_s_9	16487039	Our results suggest that globin  gene activation by heme appears to be independent of the putative HRMs  in the p45 subunit of the NF-E2 transcription factor.	transcription
79032	2	335732	6	NULL	NULL	0	NULL	statement 1	Process		is independent of					NF-E2 transcription factor	GP		HRMs in the p45 subunit		NULL		0	NULL	NULL	NULL	abs-batch0600-0619_antioxid-redox-signal_8_1-2_16487039_s_9	16487039	Our results suggest that globin  gene activation by heme appears to be independent of the putative HRMs  in the p45 subunit of the NF-E2 transcription factor.	transcription
56813	1	335733	5	NULL	NULL	0	NULL	Ngb			bind		reversibly			O2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_21_20660_s_25	15793311	Like other globins, Ngb binds O2 reversibly via an iron (Fe2+) ion of the heme group with an affinity ( P50) of about 1 Torr, which is in the range of that of Mb ( ).	transcription
56814	2	335733	5	NULL	NULL	0	NULL	Fe2+			is					iron ion					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_21_20660_s_25	15793311	Like other globins, Ngb binds O2 reversibly via an iron (Fe2+) ion of the heme group with an affinity ( P50) of about 1 Torr, which is in the range of that of Mb ( ).	transcription
56815	3	335733	5	NULL	NULL	0	NULL	statement 1			via					Fe2+					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_21_20660_s_25	15793311	Like other globins, Ngb binds O2 reversibly via an iron (Fe2+) ion of the heme group with an affinity ( P50) of about 1 Torr, which is in the range of that of Mb ( ).	transcription
56816	4	335733	5	NULL	NULL	0	NULL	Fe2+			is present in					heme group					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_21_20660_s_25	15793311	Like other globins, Ngb binds O2 reversibly via an iron (Fe2+) ion of the heme group with an affinity ( P50) of about 1 Torr, which is in the range of that of Mb ( ).	transcription
56817	5	335733	5	NULL	NULL	0	NULL	Ngb			is a type of					globin					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_21_20660_s_25	15793311	Like other globins, Ngb binds O2 reversibly via an iron (Fe2+) ion of the heme group with an affinity ( P50) of about 1 Torr, which is in the range of that of Mb ( ).	transcription
79033	1	335733	6	NULL	NULL	0	NULL	Ngb	GP		bind					O2	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_21_20660_s_25	15793311	Like other globins, Ngb binds O2 reversibly via an iron (Fe2+) ion of the heme group with an affinity ( P50) of about 1 Torr, which is in the range of that of Mb ( ).	transcription
79034	2	335733	6	NULL	NULL	0	NULL	statement 1	Process		occurs via					Fe2+	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_21_20660_s_25	15793311	Like other globins, Ngb binds O2 reversibly via an iron (Fe2+) ion of the heme group with an affinity ( P50) of about 1 Torr, which is in the range of that of Mb ( ).	transcription
56818	1	335734	5	NULL	NULL	0	NULL	GATA-1			is a type of					transcription factor					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_23_22385_s_10	15817467	ranscription factor GATA-1 recognizes conserved GATA motifs ((T/A)GATA(A/G)) in the regulatory regions of many genes encoding erythroid-restricted proteins, such as globins, heme biosynthetic enzymes, membrane proteins, and transcription factors ( ,  ).	transcription
56819	2	335734	5	NULL	NULL	0	NULL	((T/A)GATA(A/G))			is					GATA motifs					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_23_22385_s_10	15817467	ranscription factor GATA-1 recognizes conserved GATA motifs ((T/A)GATA(A/G)) in the regulatory regions of many genes encoding erythroid-restricted proteins, such as globins, heme biosynthetic enzymes, membrane proteins, and transcription factors ( ,  ).	transcription
56820	3	335734	5	NULL	NULL	0	NULL	GATA-1			recognizes					globin gene				GATA motifs	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_23_22385_s_10	15817467	ranscription factor GATA-1 recognizes conserved GATA motifs ((T/A)GATA(A/G)) in the regulatory regions of many genes encoding erythroid-restricted proteins, such as globins, heme biosynthetic enzymes, membrane proteins, and transcription factors ( ,  ).	transcription
56821	4	335734	5	NULL	NULL	0	NULL	globin gene			is present in				GATA motifs	globin gene				regulatory region	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_23_22385_s_10	15817467	ranscription factor GATA-1 recognizes conserved GATA motifs ((T/A)GATA(A/G)) in the regulatory regions of many genes encoding erythroid-restricted proteins, such as globins, heme biosynthetic enzymes, membrane proteins, and transcription factors ( ,  ).	transcription
56822	1	335735	5	NULL	NULL	0	NULL	heme			bind								NTD		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_6778_s_98	14672943	Such drastic changes in the CD spectra of His78 mutant lead us to conclude that His78 is the essential axial ligand, which is required for the specific binding of heme to the NTD, corresponding to the proximal histidine in globins.	transcription
56823	2	335735	5	NULL	NULL	0	NULL				is required for			His78		statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_6778_s_98	14672943	Such drastic changes in the CD spectra of His78 mutant lead us to conclude that His78 is the essential axial ligand, which is required for the specific binding of heme to the NTD, corresponding to the proximal histidine in globins.	transcription
79035	1	335735	6	NULL	NULL	0	NULL	Heme	GP		bind								NTD		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_6778_s_98	14672943	Such drastic changes in the CD spectra of His78 mutant lead us to conclude that His78 is the essential axial ligand, which is required for the specific binding of heme to the NTD, corresponding to the proximal histidine in globins.	transcription
56824	1	335737	5	NULL	NULL	0	NULL	heme			bind					globin					NULL		0	NULL	NULL	NULL	gw60_embo_22_8_1824_s_198	12682015	Also similar to TipAS antibiotic binding, heme binding to globins induces the folding of additional alpha-helices that are in contact with the ligand ( Eliezer and Wright, 1996;  Wakasugi  et al., 1997;  Eliezer  et al., 1998).	transcription
56825	2	335737	5	NULL	NULL	0	NULL	statement 1			induce							folding of	alpha-helices		NULL		0	NULL	NULL	NULL	gw60_embo_22_8_1824_s_198	12682015	Also similar to TipAS antibiotic binding, heme binding to globins induces the folding of additional alpha-helices that are in contact with the ligand ( Eliezer and Wright, 1996;  Wakasugi  et al., 1997;  Eliezer  et al., 1998).	transcription
79036	1	335737	6	NULL	NULL	0	NULL	heme	GP		bind					globin	GP				NULL		0	NULL	NULL	NULL	gw60_embo_22_8_1824_s_198	12682015	Also similar to TipAS antibiotic binding, heme binding to globins induces the folding of additional alpha-helices that are in contact with the ligand ( Eliezer and Wright, 1996;  Wakasugi  et al., 1997;  Eliezer  et al., 1998).	transcription
79037	1	335739	6	NULL	NULL	0	NULL				bind			beta Lys-66		heme			propionic acid group of pyrrole IV		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_27_16998_s_263	9642264	Additional stabilization of the hemin in  C. lacteus globins is provided by the interaction of residue Lys-47 (E10) corresponding to human beta Lys-66 (E10) which is known to form an electrostatic link with the propionic acid group of pyrrole IV of the heme ( 26).	transcription
56826	1	335740	5	NULL	NULL	0	NULL	globin			does not leave					ribosome					NULL		0	NULL	NULL	NULL	gw60_cell_108_5_591_s_51	11893330	Since competence to bind the heme group requires formation of the heme binding site, and since folding in the exit tunnel is precluded by its small size, this suggests that globin cannot leave the ribosome via the exit tunnel.	transcription
56827	2	335740	5	NULL	NULL	0	NULL	statement 1			via					exit tunnel					NULL		0	NULL	NULL	NULL	gw60_cell_108_5_591_s_51	11893330	Since competence to bind the heme group requires formation of the heme binding site, and since folding in the exit tunnel is precluded by its small size, this suggests that globin cannot leave the ribosome via the exit tunnel.	transcription
79038	1	335740	6	NULL	NULL	0	NULL	globin	GP		cannot leave					ribosome	CellComponent				NULL		0	NULL	NULL	NULL	gw60_cell_108_5_591_s_51	11893330	Since competence to bind the heme group requires formation of the heme binding site, and since folding in the exit tunnel is precluded by its small size, this suggests that globin cannot leave the ribosome via the exit tunnel.	transcription
79039	2	335740	6	NULL	NULL	0	NULL	statement 1	Process		occurs via					exit tunnel					NULL		0	NULL	NULL	NULL	gw60_cell_108_5_591_s_51	11893330	Since competence to bind the heme group requires formation of the heme binding site, and since folding in the exit tunnel is precluded by its small size, this suggests that globin cannot leave the ribosome via the exit tunnel.	transcription
56828	1	335741	5	NULL	NULL	0	NULL	alpha-globin chains			bind					ribosome					NULL		0	NULL	NULL	NULL	gw60_annrevbiochem_70_0_603_s_305	11395418	For instance, ribosome-bound alpha-globin chains can bind heme after synthesis of only 86 amino acids, possibly reflecting the formation of a folded heme-binding pocket ( 156).	transcription
56829	2	335741	5	NULL	NULL	0	NULL	statement 1			bind					heme					NULL		0	NULL	NULL	NULL	gw60_annrevbiochem_70_0_603_s_305	11395418	For instance, ribosome-bound alpha-globin chains can bind heme after synthesis of only 86 amino acids, possibly reflecting the formation of a folded heme-binding pocket ( 156).	transcription
79040	1	335741	6	NULL	NULL	0	NULL	ribosome	CellComponent		bind					alpha-globin	GP				NULL		0	NULL	NULL	NULL	gw60_annrevbiochem_70_0_603_s_305	11395418	For instance, ribosome-bound alpha-globin chains can bind heme after synthesis of only 86 amino acids, possibly reflecting the formation of a folded heme-binding pocket ( 156).	transcription
79041	2	335741	6	NULL	NULL	0	NULL	statement 1	Process		bind					Heme	GP				NULL		0	NULL	NULL	NULL	gw60_annrevbiochem_70_0_603_s_305	11395418	For instance, ribosome-bound alpha-globin chains can bind heme after synthesis of only 86 amino acids, possibly reflecting the formation of a folded heme-binding pocket ( 156).	transcription
79042	1	335742	6	NULL	NULL	0	NULL	Heme	GP		bind								beta chain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10130_s_9	8626572	These results  indicate that in human hemoglobin the heme-globin linkage in the alpha   chains is stabilized by interactions between unlike chains at the  alpha beta   interface, whereas heme binding to  the beta  chains is stabilized by interactions at the  alpha beta   interface.	transcription
79043	2	335742	6	NULL	NULL	0	NULL	statement 1	Process		is stablized by								alpha beta interface		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10130_s_9	8626572	These results  indicate that in human hemoglobin the heme-globin linkage in the alpha   chains is stabilized by interactions between unlike chains at the  alpha beta   interface, whereas heme binding to  the beta  chains is stabilized by interactions at the  alpha beta   interface.	transcription
56830	1	335743	5	NULL	NULL	0	NULL	heme			bind					globin					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_40_24564_s_84	8798719	The side chain of Leu-beta88 (F4) contacts the heme side chain ( 13), and binding of heme to globin involves a specific stereochemical fit that helps stabilize tertiary conformation of the subunit.	transcription
56831	1	335746	5	NULL	NULL	0	NULL	Me2SO			mediates					beta-globin mRNA		increase in			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_5358_s_144	9478996	Inhibition of Serine/hreonine Phosphorylation Also Inhibits the Me2SO- mediated Increase in beta -Globin and ALAS-E mRNA Levels and Heme Content-- To examine the effect of inhibition of serine/threonine phosphorylation on erythroid differentiation, the effect of 2-AP on Me2SO-mediated induction of  beta-globin and  ALAS-E mRNAs and heme content was examined.	transcription
56832	2	335746	5	NULL	NULL	0	NULL	Me2SO			mediates					ALAS-E mRNA		increase in			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_5358_s_144	9478996	Inhibition of Serine/hreonine Phosphorylation Also Inhibits the Me2SO- mediated Increase in beta -Globin and ALAS-E mRNA Levels and Heme Content-- To examine the effect of inhibition of serine/threonine phosphorylation on erythroid differentiation, the effect of 2-AP on Me2SO-mediated induction of  beta-globin and  ALAS-E mRNAs and heme content was examined.	transcription
56833	3	335746	5	NULL	NULL	0	NULL	Me2SO			mediates					heme		increase in			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_5358_s_144	9478996	Inhibition of Serine/hreonine Phosphorylation Also Inhibits the Me2SO- mediated Increase in beta -Globin and ALAS-E mRNA Levels and Heme Content-- To examine the effect of inhibition of serine/threonine phosphorylation on erythroid differentiation, the effect of 2-AP on Me2SO-mediated induction of  beta-globin and  ALAS-E mRNAs and heme content was examined.	transcription
56834	4	335746	5	NULL	NULL	0	NULL	serine/threonine		inhibition of;;phosphorylation of	inhibits					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_5358_s_144	9478996	Inhibition of Serine/hreonine Phosphorylation Also Inhibits the Me2SO- mediated Increase in beta -Globin and ALAS-E mRNA Levels and Heme Content-- To examine the effect of inhibition of serine/threonine phosphorylation on erythroid differentiation, the effect of 2-AP on Me2SO-mediated induction of  beta-globin and  ALAS-E mRNAs and heme content was examined.	transcription
56835	5	335746	5	NULL	NULL	0	NULL	serine/threonine		inhibition of;;phosphorylation of	inhibits					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_5358_s_144	9478996	Inhibition of Serine/hreonine Phosphorylation Also Inhibits the Me2SO- mediated Increase in beta -Globin and ALAS-E mRNA Levels and Heme Content-- To examine the effect of inhibition of serine/threonine phosphorylation on erythroid differentiation, the effect of 2-AP on Me2SO-mediated induction of  beta-globin and  ALAS-E mRNAs and heme content was examined.	transcription
56836	6	335746	5	NULL	NULL	0	NULL	serine/threonine		inhibition of;;phosphorylation of	inhibits					statement 3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_5358_s_144	9478996	Inhibition of Serine/hreonine Phosphorylation Also Inhibits the Me2SO- mediated Increase in beta -Globin and ALAS-E mRNA Levels and Heme Content-- To examine the effect of inhibition of serine/threonine phosphorylation on erythroid differentiation, the effect of 2-AP on Me2SO-mediated induction of  beta-globin and  ALAS-E mRNAs and heme content was examined.	transcription
79044	1	335746	6	NULL	NULL	0	NULL	Me2SO	Chemical		mediates					beta-globin	GP	increase in			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_5358_s_144	9478996	Inhibition of Serine/hreonine Phosphorylation Also Inhibits the Me2SO- mediated Increase in beta -Globin and ALAS-E mRNA Levels and Heme Content-- To examine the effect of inhibition of serine/threonine phosphorylation on erythroid differentiation, the effect of 2-AP on Me2SO-mediated induction of  beta-globin and  ALAS-E mRNAs and heme content was examined.	transcription
79045	2	335746	6	NULL	NULL	0	NULL	Me2SO	Chemical		mediates					ALAS-E mRNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_5358_s_144	9478996	Inhibition of Serine/hreonine Phosphorylation Also Inhibits the Me2SO- mediated Increase in beta -Globin and ALAS-E mRNA Levels and Heme Content-- To examine the effect of inhibition of serine/threonine phosphorylation on erythroid differentiation, the effect of 2-AP on Me2SO-mediated induction of  beta-globin and  ALAS-E mRNAs and heme content was examined.	transcription
79046	3	335746	6	NULL	NULL	0	NULL	Me2SO	Chemical		mediates					Heme	GP	increase in			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_5358_s_144	9478996	Inhibition of Serine/hreonine Phosphorylation Also Inhibits the Me2SO- mediated Increase in beta -Globin and ALAS-E mRNA Levels and Heme Content-- To examine the effect of inhibition of serine/threonine phosphorylation on erythroid differentiation, the effect of 2-AP on Me2SO-mediated induction of  beta-globin and  ALAS-E mRNAs and heme content was examined.	transcription
79047	4	335746	6	NULL	NULL	0	NULL	Serine/hreonine	AminoAcid	inhibition of;; phosphorylation of 	inhibits					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_5358_s_144	9478996	Inhibition of Serine/hreonine Phosphorylation Also Inhibits the Me2SO- mediated Increase in beta -Globin and ALAS-E mRNA Levels and Heme Content-- To examine the effect of inhibition of serine/threonine phosphorylation on erythroid differentiation, the effect of 2-AP on Me2SO-mediated induction of  beta-globin and  ALAS-E mRNAs and heme content was examined.	transcription
79048	5	335746	6	NULL	NULL	0	NULL	Serine/hreonine	AminoAcid	inhibition of;; phosphorylation of 	inhibits					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_5358_s_144	9478996	Inhibition of Serine/hreonine Phosphorylation Also Inhibits the Me2SO- mediated Increase in beta -Globin and ALAS-E mRNA Levels and Heme Content-- To examine the effect of inhibition of serine/threonine phosphorylation on erythroid differentiation, the effect of 2-AP on Me2SO-mediated induction of  beta-globin and  ALAS-E mRNAs and heme content was examined.	transcription
79049	6	335746	6	NULL	NULL	0	NULL	Serine/hreonine	AminoAcid	inhibition of;; phosphorylation of 	inhibits					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_5358_s_144	9478996	Inhibition of Serine/hreonine Phosphorylation Also Inhibits the Me2SO- mediated Increase in beta -Globin and ALAS-E mRNA Levels and Heme Content-- To examine the effect of inhibition of serine/threonine phosphorylation on erythroid differentiation, the effect of 2-AP on Me2SO-mediated induction of  beta-globin and  ALAS-E mRNAs and heme content was examined.	transcription
56837	1	335747	5	NULL	NULL	0	NULL	heme			stimulates					globin gene		transcription of			NULL		0	NULL	NULL	NULL	gw70_annurevnutr_24_0_105_s_458	15189115	Numerous reports indicate that heme stimulates globin gene transcription and is  probably involved in promoting some other aspects of erythroid differentiation ( 105).	transcription
56838	2	335747	5	NULL	NULL	0	NULL	heme			promotes		probably			erythroid		differentiation of			NULL		0	NULL	NULL	NULL	gw70_annurevnutr_24_0_105_s_458	15189115	Numerous reports indicate that heme stimulates globin gene transcription and is  probably involved in promoting some other aspects of erythroid differentiation ( 105).	transcription
56839	1	335748	5	NULL	NULL	0	NULL	heme			bind					HRI					NULL	erythroid cells	NULL	NULL	NULL	NULL	gw70_annurevnutr_24_0_105_s_469	15189115	Heme binding to  HRI inhibits the phosphorylation of eIF-2  by HRI, resulting in an efficient translation  of globin and probably other proteins in erythroid cells ( 23, 113).	transcription
56840	2	335748	5	NULL	NULL	0	NULL	HRI			phosphorylates					eIF-2					NULL	erythroid cells	NULL	NULL	NULL	NULL	gw70_annurevnutr_24_0_105_s_469	15189115	Heme binding to  HRI inhibits the phosphorylation of eIF-2  by HRI, resulting in an efficient translation  of globin and probably other proteins in erythroid cells ( 23, 113).	transcription
56841	3	335748	5	NULL	NULL	0	NULL	statement 1			inhibits					statement 2					NULL	erythroid cells	NULL	NULL	NULL	NULL	gw70_annurevnutr_24_0_105_s_469	15189115	Heme binding to  HRI inhibits the phosphorylation of eIF-2  by HRI, resulting in an efficient translation  of globin and probably other proteins in erythroid cells ( 23, 113).	transcription
56842	4	335748	5	NULL	NULL	0	NULL	statement 3			results in					globin		efficient translation			NULL	erythroid cells	0	NULL	NULL	NULL	gw70_annurevnutr_24_0_105_s_469	15189115	Heme binding to  HRI inhibits the phosphorylation of eIF-2  by HRI, resulting in an efficient translation  of globin and probably other proteins in erythroid cells ( 23, 113).	transcription
79050	1	335748	6	NULL	NULL	0	NULL	Heme	GP		bind					HRI	GP				NULL		0	NULL	NULL	NULL	gw70_annurevnutr_24_0_105_s_469	15189115	Heme binding to  HRI inhibits the phosphorylation of eIF-2  by HRI, resulting in an efficient translation  of globin and probably other proteins in erythroid cells ( 23, 113).	transcription
56843	1	335749	5	NULL	NULL	0	NULL	HRI			regulates					globin		synthesis of			NULL	developing reticulocytes	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_21_20331_s_312	15788408	HRI regulates globin synthesis to match heme availability in developing reticulocytes ( ) and may regulate eIF2alpha phosphorylation in response to certain oxidative stresses.	transcription
56844	2	335749	5	NULL	NULL	0	NULL	statement 1			match					heme		availability of			NULL	developing reticulocytes	0	NULL	NULL	NULL	gw70_jbiolchem_280_21_20331_s_312	15788408	HRI regulates globin synthesis to match heme availability in developing reticulocytes ( ) and may regulate eIF2alpha phosphorylation in response to certain oxidative stresses.	transcription
56845	3	335749	5	NULL	NULL	0	NULL	HRI			regulates		may			eIF2alpha		phosphorylation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_21_20331_s_312	15788408	HRI regulates globin synthesis to match heme availability in developing reticulocytes ( ) and may regulate eIF2alpha phosphorylation in response to certain oxidative stresses.	transcription
56846	4	335749	5	NULL	NULL	0	NULL	statement 3			in response to					oxidative stress					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_21_20331_s_312	15788408	HRI regulates globin synthesis to match heme availability in developing reticulocytes ( ) and may regulate eIF2alpha phosphorylation in response to certain oxidative stresses.	transcription
79051	1	335749	6	NULL	NULL	0	NULL	HRI	GP		regulates					globin	GP	synthesis of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_21_20331_s_312	15788408	HRI regulates globin synthesis to match heme availability in developing reticulocytes ( ) and may regulate eIF2alpha phosphorylation in response to certain oxidative stresses.	transcription
79052	2	335749	6	NULL	NULL	0	NULL	HRI	GP		regulates		may			eIF2alpha	GP	phosphorylation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_21_20331_s_312	15788408	HRI regulates globin synthesis to match heme availability in developing reticulocytes ( ) and may regulate eIF2alpha phosphorylation in response to certain oxidative stresses.	transcription
56847	1	335750	5	NULL	NULL	0	NULL	heme			controls					muLCR-beta-globin promoter reporter gene					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_9	14660636	The control of the muLCR-beta-globin promoter reporter gene by heme was dependent on DNase I-hypersensitive site 2 (HS2), which contains MARE.	transcription
56848	2	335750	5	NULL	NULL	0	NULL	statement 1			is dependent on					DNase I				HS2	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_9	14660636	The control of the muLCR-beta-globin promoter reporter gene by heme was dependent on DNase I-hypersensitive site 2 (HS2), which contains MARE.	transcription
56849	3	335750	5	NULL	NULL	0	NULL	DNase I			contains				HS2					MARE	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_9	14660636	The control of the muLCR-beta-globin promoter reporter gene by heme was dependent on DNase I-hypersensitive site 2 (HS2), which contains MARE.	transcription
56850	4	335750	5	NULL	NULL	0	NULL	HS2			is					hypersensitive site 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_9	14660636	The control of the muLCR-beta-globin promoter reporter gene by heme was dependent on DNase I-hypersensitive site 2 (HS2), which contains MARE.	transcription
56851	1	335751	5	NULL	NULL	0	NULL	AHSP			bind					Fe(II) alphaHb					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_43_32611_s_5	16901899	Binding of AHSP to Fe(II) alphaHb induces an unusual configuration in which the F helix of the globin becomes disordered and the heme ring becomes solvent-exposed.	transcription
56852	2	335751	5	NULL	NULL	0	NULL	globin			becomes			F helix		disordered					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_43_32611_s_5	16901899	Binding of AHSP to Fe(II) alphaHb induces an unusual configuration in which the F helix of the globin becomes disordered and the heme ring becomes solvent-exposed.	transcription
56853	3	335751	5	NULL	NULL	0	NULL	heme ring			is exposed to					solvent					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_43_32611_s_5	16901899	Binding of AHSP to Fe(II) alphaHb induces an unusual configuration in which the F helix of the globin becomes disordered and the heme ring becomes solvent-exposed.	transcription
56854	4	335751	5	NULL	NULL	0	NULL	statement 1			leads to					statement 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_43_32611_s_5	16901899	Binding of AHSP to Fe(II) alphaHb induces an unusual configuration in which the F helix of the globin becomes disordered and the heme ring becomes solvent-exposed.	transcription
56855	5	335751	5	NULL	NULL	0	NULL	statement 1			leads to					statement 3					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_43_32611_s_5	16901899	Binding of AHSP to Fe(II) alphaHb induces an unusual configuration in which the F helix of the globin becomes disordered and the heme ring becomes solvent-exposed.	transcription
79053	1	335751	6	NULL	NULL	0	NULL	AHSP	GP		bind					Fe(II) alphaHb	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_43_32611_s_5	16901899	Binding of AHSP to Fe(II) alphaHb induces an unusual configuration in which the F helix of the globin becomes disordered and the heme ring becomes solvent-exposed.	transcription
56856	1	335752	5	NULL	NULL	0	NULL	AHSP			bind					apo alpha globin protein					NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbiolchem_281_43_32611_s_337	16901899	For example, AHSP binds apo (non heme-bound) alpha globin protein  in vitro ( ) and facilitates its folding and expression in  Escherichia coli and in eukaryotic cells ( ,  ).	transcription
56857	2	335752	5	NULL	NULL	0	NULL	statement 1			facilitates					apo alpha globin protein		folding of			NULL	in vitro	0	NULL	NULL	NULL	gw70_jbiolchem_281_43_32611_s_337	16901899	For example, AHSP binds apo (non heme-bound) alpha globin protein  in vitro ( ) and facilitates its folding and expression in  Escherichia coli and in eukaryotic cells ( ,  ).	transcription
56858	3	335752	5	NULL	NULL	0	NULL	statement 1			facilitates					apo alpha globin protein		expression of			NULL	Escherichia coli, eukaryotic cells	0	NULL	NULL	NULL	gw70_jbiolchem_281_43_32611_s_337	16901899	For example, AHSP binds apo (non heme-bound) alpha globin protein  in vitro ( ) and facilitates its folding and expression in  Escherichia coli and in eukaryotic cells ( ,  ).	transcription
79054	1	335752	6	NULL	NULL	0	NULL	AHSP	GP		bind					apo alpha globin protein	GP				NULL	in vitro	0	NULL	NULL	NULL	gw70_jbiolchem_281_43_32611_s_337	16901899	For example, AHSP binds apo (non heme-bound) alpha globin protein  in vitro ( ) and facilitates its folding and expression in  Escherichia coli and in eukaryotic cells ( ,  ).	transcription
56859	1	335753	5	NULL	NULL	0	NULL	RsbR			does not bind					heme					NULL		0	NULL	NULL	NULL	gw70_pnas_102_48_17320_s_127	16301540	Despite the globin fold of N-RsbR, there is no evidence, through spectroscopy or careful inspection of the electron density maps of N-RsbR, for heme binding by RsbR.	transcription
56860	1	335754	5	NULL	NULL	0	NULL	Bach1			displaced from					beta-globin				locus control region	NULL	murine erythroleukemia cells	NULL	NULL	NULL	NULL	gw70_pnas_101_6_1461_s_10	14747657	Heme also promotes displacement of Bach1 from the beta-globin locus control region without affecting MafK binding in murine erythroleukemia cells.	transcription
56861	2	335754	5	NULL	NULL	0	NULL	heme			promotes					statement 1					NULL	murine erythroleukemia cells	0	NULL	NULL	NULL	gw70_pnas_101_6_1461_s_10	14747657	Heme also promotes displacement of Bach1 from the beta-globin locus control region without affecting MafK binding in murine erythroleukemia cells.	transcription
56862	3	335754	5	NULL	NULL	0	NULL	statement 2			does not affect					MafK		binding of			NULL	murine erythroleukemia cells	0	NULL	NULL	NULL	gw70_pnas_101_6_1461_s_10	14747657	Heme also promotes displacement of Bach1 from the beta-globin locus control region without affecting MafK binding in murine erythroleukemia cells.	transcription
79055	1	335754	6	NULL	NULL	0	NULL	heme	GP		promotes					Bach1	GP	displacement of			NULL		0	NULL	NULL	NULL	gw70_pnas_101_6_1461_s_10	14747657	Heme also promotes displacement of Bach1 from the beta-globin locus control region without affecting MafK binding in murine erythroleukemia cells.	transcription
79056	2	335754	6	NULL	NULL	NULL	NULL	statement 1	Process		does not affect					MafK	GP	binding of 			NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_6_1461_s_10	14747657	Heme also promotes displacement of Bach1 from the beta-globin locus control region without affecting MafK binding in murine erythroleukemia cells.	transcription
56863	1	335755	5	NULL	NULL	0	NULL	Bach1			departs from									LCR	NULL		0	NULL	NULL	NULL	gw70_pnas_101_6_1461_s_194	14747657	These results indicate that the heme-mediated departure of Bach1 from the LCR is not sufficient for the activation of beta-globin expression or the induction of MEL cell differentiation.	transcription
56864	2	335755	5	NULL	NULL	0	NULL	heme			mediates					statement 1					NULL		0	NULL	NULL	NULL	gw70_pnas_101_6_1461_s_194	14747657	These results indicate that the heme-mediated departure of Bach1 from the LCR is not sufficient for the activation of beta-globin expression or the induction of MEL cell differentiation.	transcription
56865	3	335755	5	NULL	NULL	0	NULL	statement 2			is not sufficient for					beta-globin		activation of;;expression of			NULL		0	NULL	NULL	NULL	gw70_pnas_101_6_1461_s_194	14747657	These results indicate that the heme-mediated departure of Bach1 from the LCR is not sufficient for the activation of beta-globin expression or the induction of MEL cell differentiation.	transcription
56866	4	335755	5	NULL	NULL	0	NULL	statement 2			is not sufficient for					MEL cell		induction of;;differentiation of			NULL		0	NULL	NULL	NULL	gw70_pnas_101_6_1461_s_194	14747657	These results indicate that the heme-mediated departure of Bach1 from the LCR is not sufficient for the activation of beta-globin expression or the induction of MEL cell differentiation.	transcription
79057	1	335755	6	NULL	NULL	0	NULL	Bach1	GP		is removed from					LCR	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_6_1461_s_194	14747657	These results indicate that the heme-mediated departure of Bach1 from the LCR is not sufficient for the activation of beta-globin expression or the induction of MEL cell differentiation.	transcription
79058	2	335755	6	NULL	NULL	0	NULL	statement 1	Process		is dependent on					Heme	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_6_1461_s_194	14747657	These results indicate that the heme-mediated departure of Bach1 from the LCR is not sufficient for the activation of beta-globin expression or the induction of MEL cell differentiation.	transcription
79059	3	335755	6	NULL	NULL	0	NULL	statement 1	Process		is not sufficient for					beta-globin	GP	activation of;; expression of			NULL		0	NULL	NULL	NULL	gw70_pnas_101_6_1461_s_194	14747657	These results indicate that the heme-mediated departure of Bach1 from the LCR is not sufficient for the activation of beta-globin expression or the induction of MEL cell differentiation.	transcription
79060	4	335755	6	NULL	NULL	0	NULL	statement 1	Process		is not sufficient for					MEL cell	Process	differentiation of			NULL		0	NULL	NULL	NULL	gw70_pnas_101_6_1461_s_194	14747657	These results indicate that the heme-mediated departure of Bach1 from the LCR is not sufficient for the activation of beta-globin expression or the induction of MEL cell differentiation.	transcription
56867	1	335757	5	NULL	NULL	0	NULL	heme			regulates					HO-1		expression of			NULL		0	NULL	NULL	NULL	abs-batch0600-0619_antioxid-redox-signal_8_1-2_16487043_s_8	16487043	By modulating the equilibrium  of the small Maf heterodimer network, heme regulates expression of the  cytoprotective enzyme HO-1 during the stress response and of beta-globin  during erythroid differentiation.	transcription
56868	2	335757	5	NULL	NULL	0	NULL	HO-1			is a type of					cytoprotective enzyme					NULL		0	NULL	NULL	NULL	abs-batch0600-0619_antioxid-redox-signal_8_1-2_16487043_s_8	16487043	By modulating the equilibrium  of the small Maf heterodimer network, heme regulates expression of the  cytoprotective enzyme HO-1 during the stress response and of beta-globin  during erythroid differentiation.	transcription
56869	3	335757	5	NULL	NULL	0	NULL	Maf heterodimer network		modulating the equilibrium of;;small	leads to					statement 1					NULL		0	NULL	NULL	NULL	abs-batch0600-0619_antioxid-redox-signal_8_1-2_16487043_s_8	16487043	By modulating the equilibrium  of the small Maf heterodimer network, heme regulates expression of the  cytoprotective enzyme HO-1 during the stress response and of beta-globin  during erythroid differentiation.	transcription
56870	4	335757	5	NULL	NULL	0	NULL	statement 1			occurs during					stress response					NULL		0	NULL	NULL	NULL	abs-batch0600-0619_antioxid-redox-signal_8_1-2_16487043_s_8	16487043	By modulating the equilibrium  of the small Maf heterodimer network, heme regulates expression of the  cytoprotective enzyme HO-1 during the stress response and of beta-globin  during erythroid differentiation.	transcription
56871	5	335757	5	NULL	NULL	0	NULL	heme			regulates					beta-globin		expression of			NULL		0	NULL	NULL	NULL	abs-batch0600-0619_antioxid-redox-signal_8_1-2_16487043_s_8	16487043	By modulating the equilibrium  of the small Maf heterodimer network, heme regulates expression of the  cytoprotective enzyme HO-1 during the stress response and of beta-globin  during erythroid differentiation.	transcription
56872	6	335757	5	NULL	NULL	0	NULL	statement 5			occurs during					erythroid		differentiation of			NULL		0	NULL	NULL	NULL	abs-batch0600-0619_antioxid-redox-signal_8_1-2_16487043_s_8	16487043	By modulating the equilibrium  of the small Maf heterodimer network, heme regulates expression of the  cytoprotective enzyme HO-1 during the stress response and of beta-globin  during erythroid differentiation.	transcription
56873	7	335757	5	NULL	NULL	0	NULL	Maf heterodimer network		modulating the equilibrium of;;small	leads to					statement 5					NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_antioxid-redox-signal_8_1-2_16487043_s_8	16487043	By modulating the equilibrium  of the small Maf heterodimer network, heme regulates expression of the  cytoprotective enzyme HO-1 during the stress response and of beta-globin  during erythroid differentiation.	transcription
79061	1	335757	6	NULL	NULL	0	NULL	heme	GP		regulates					HO-1	GP	expression of			NULL		0	NULL	NULL	NULL	abs-batch0600-0619_antioxid-redox-signal_8_1-2_16487043_s_8	16487043	By modulating the equilibrium  of the small Maf heterodimer network, heme regulates expression of the  cytoprotective enzyme HO-1 during the stress response and of beta-globin  during erythroid differentiation.	transcription
79062	2	335757	6	NULL	NULL	0	NULL	HO-1	GP		is a type of					cytoprotective enzyme					NULL		0	NULL	NULL	NULL	abs-batch0600-0619_antioxid-redox-signal_8_1-2_16487043_s_8	16487043	By modulating the equilibrium  of the small Maf heterodimer network, heme regulates expression of the  cytoprotective enzyme HO-1 during the stress response and of beta-globin  during erythroid differentiation.	transcription
79063	3	335757	6	NULL	NULL	0	NULL	heme	GP		regulates					beta-globin	GP	expression of			NULL		0	NULL	NULL	NULL	abs-batch0600-0619_antioxid-redox-signal_8_1-2_16487043_s_8	16487043	By modulating the equilibrium  of the small Maf heterodimer network, heme regulates expression of the  cytoprotective enzyme HO-1 during the stress response and of beta-globin  during erythroid differentiation.	transcription
79064	4	335757	6	NULL	NULL	0	NULL	statement 3	GP		occurs during					erythroid differentiation	Process				NULL		0	NULL	NULL	NULL	abs-batch0600-0619_antioxid-redox-signal_8_1-2_16487043_s_8	16487043	By modulating the equilibrium  of the small Maf heterodimer network, heme regulates expression of the  cytoprotective enzyme HO-1 during the stress response and of beta-globin  during erythroid differentiation.	transcription
56874	1	335758	5	NULL	NULL	0	NULL	heme			controls					microLCR-beta-globin promoter reporter gene					NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_279_7_14660636_s_9	14660636	The control of the microLCR-beta-globin  promoter reporter gene by heme was dependent on DNase I-hypersensitive  site 2 (HS2), which contains MARE.	transcription
56875	2	335758	5	NULL	NULL	0	NULL	statement 1			is dependent on					DNase I				HS2	NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_279_7_14660636_s_9	14660636	The control of the microLCR-beta-globin  promoter reporter gene by heme was dependent on DNase I-hypersensitive  site 2 (HS2), which contains MARE.	transcription
56876	3	335758	5	NULL	NULL	0	NULL	DNase I			contains				HS2					MARE	NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_279_7_14660636_s_9	14660636	The control of the microLCR-beta-globin  promoter reporter gene by heme was dependent on DNase I-hypersensitive  site 2 (HS2), which contains MARE.	transcription
56877	4	335758	5	NULL	NULL	0	NULL	HS2			is					hypersensitive site 2					NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_279_7_14660636_s_9	14660636	The control of the microLCR-beta-globin  promoter reporter gene by heme was dependent on DNase I-hypersensitive  site 2 (HS2), which contains MARE.	transcription
79065	1	335758	6	NULL	NULL	0	NULL	Heme	GP		controls					microLCR-beta-globin promoter	GP				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_279_7_14660636_s_9	14660636	The control of the microLCR-beta-globin  promoter reporter gene by heme was dependent on DNase I-hypersensitive  site 2 (HS2), which contains MARE.	transcription
56878	1	335759	5	NULL	NULL	0	NULL	heme			split from					globin					NULL		0	NULL	NULL	NULL	abs-batch0650-0679_zh-evol-biokhim-fiziol_13_2_868393_s_4	868393	It was shown that splitting of heme from  the globin results in an increase of the area occupied by the molecule  on the phase boarderline from 36-10(2) to 47-10(2) A2.	transcription
57104	1	335761	5	NULL	NULL	0	NULL	globin mRNA		regulation of;;translation of	is dependent on					heme					NULL		0	NULL	NULL	NULL	gw70_embo_23_13_2544_s_260	15175654	This type of regulation, together with  the heme-dependent regulation of globin mRNA translation (  et al), may be important in avoiding toxicity due to the pro-oxidant nature of free heme  during erythroid differentiation, since such a mechanistic link furthers the incorporation  of heme into hemoglobin.	transcription
57105	2	335761	5	NULL	NULL	0	NULL	heme			is incorporated into					hemoglobin					NULL		0	NULL	NULL	NULL	gw70_embo_23_13_2544_s_260	15175654	This type of regulation, together with  the heme-dependent regulation of globin mRNA translation (  et al), may be important in avoiding toxicity due to the pro-oxidant nature of free heme  during erythroid differentiation, since such a mechanistic link furthers the incorporation  of heme into hemoglobin.	transcription
56879	1	335762	5	NULL	NULL	0	NULL	AHSP			bind					oxy-alphaHb		free			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_43_32611_s_26	16901899	The initial binding of AHSP to free oxy-alphaHb causes disordering of the globin F helix, movement of the heme group, displacement of the F8 histidine, coordination of the Fe(II) heme iron by the distal histidine (E7), and binding of O2 to the proximal side of the heme group ( ).	transcription
56880	2	335762	5	NULL	NULL	0	NULL	statement 1			causes					globin		disordering of	F helix		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_43_32611_s_26	16901899	The initial binding of AHSP to free oxy-alphaHb causes disordering of the globin F helix, movement of the heme group, displacement of the F8 histidine, coordination of the Fe(II) heme iron by the distal histidine (E7), and binding of O2 to the proximal side of the heme group ( ).	transcription
56881	3	335762	5	NULL	NULL	0	NULL	statement 1			causes					heme group		movement of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_43_32611_s_26	16901899	The initial binding of AHSP to free oxy-alphaHb causes disordering of the globin F helix, movement of the heme group, displacement of the F8 histidine, coordination of the Fe(II) heme iron by the distal histidine (E7), and binding of O2 to the proximal side of the heme group ( ).	transcription
56882	4	335762	5	NULL	NULL	0	NULL	statement 1			causes					F8 histidine		displacement of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_43_32611_s_26	16901899	The initial binding of AHSP to free oxy-alphaHb causes disordering of the globin F helix, movement of the heme group, displacement of the F8 histidine, coordination of the Fe(II) heme iron by the distal histidine (E7), and binding of O2 to the proximal side of the heme group ( ).	transcription
56883	5	335762	5	NULL	NULL	0	NULL	Fe(II) heme iron			is coordinated by					histidine (E7)		distal			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_43_32611_s_26	16901899	The initial binding of AHSP to free oxy-alphaHb causes disordering of the globin F helix, movement of the heme group, displacement of the F8 histidine, coordination of the Fe(II) heme iron by the distal histidine (E7), and binding of O2 to the proximal side of the heme group ( ).	transcription
56884	6	335762	5	NULL	NULL	0	NULL	statement 1			causes					statement 5					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_43_32611_s_26	16901899	The initial binding of AHSP to free oxy-alphaHb causes disordering of the globin F helix, movement of the heme group, displacement of the F8 histidine, coordination of the Fe(II) heme iron by the distal histidine (E7), and binding of O2 to the proximal side of the heme group ( ).	transcription
56885	7	335762	5	NULL	NULL	0	NULL	O2			bind					heme group		proximal side of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_43_32611_s_26	16901899	The initial binding of AHSP to free oxy-alphaHb causes disordering of the globin F helix, movement of the heme group, displacement of the F8 histidine, coordination of the Fe(II) heme iron by the distal histidine (E7), and binding of O2 to the proximal side of the heme group ( ).	transcription
56886	8	335762	5	NULL	NULL	0	NULL	statement 1			causes					statement 7					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_43_32611_s_26	16901899	The initial binding of AHSP to free oxy-alphaHb causes disordering of the globin F helix, movement of the heme group, displacement of the F8 histidine, coordination of the Fe(II) heme iron by the distal histidine (E7), and binding of O2 to the proximal side of the heme group ( ).	transcription
79066	1	335762	6	NULL	NULL	0	NULL	AHSP	GP		bind					oxy-alphaHb	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_43_32611_s_26	16901899	The initial binding of AHSP to free oxy-alphaHb causes disordering of the globin F helix, movement of the heme group, displacement of the F8 histidine, coordination of the Fe(II) heme iron by the distal histidine (E7), and binding of O2 to the proximal side of the heme group ( ).	transcription
56887	1	335763	5	NULL	NULL	0	NULL	rHbs		high soluble expression of	requires					heme		excess of			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_640_s_206	9925594	Since very high soluble expression of rHbs always required a >2.5-fold molar excess of heme, this excess may be required for sufficient diffusion across the cell membrane to maintain an intracellular heme concentration high enough to drive the bimolecular reaction of heme with globin.	transcription
56888	2	335763	5	NULL	NULL	0	NULL	heme		excess	is diffussed across					cell membrane					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_640_s_206	9925594	Since very high soluble expression of rHbs always required a >2.5-fold molar excess of heme, this excess may be required for sufficient diffusion across the cell membrane to maintain an intracellular heme concentration high enough to drive the bimolecular reaction of heme with globin.	transcription
56890	3	335763	5	NULL	NULL	0	NULL	statement 2			maintains					heme		high concentration of;;intracellular			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_640_s_206	9925594	Since very high soluble expression of rHbs always required a >2.5-fold molar excess of heme, this excess may be required for sufficient diffusion across the cell membrane to maintain an intracellular heme concentration high enough to drive the bimolecular reaction of heme with globin.	transcription
56891	4	335763	5	NULL	NULL	0	NULL	heme			bind					globin					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_640_s_206	9925594	Since very high soluble expression of rHbs always required a >2.5-fold molar excess of heme, this excess may be required for sufficient diffusion across the cell membrane to maintain an intracellular heme concentration high enough to drive the bimolecular reaction of heme with globin.	transcription
56892	5	335763	5	NULL	NULL	0	NULL	statement 3			drives					statement 4					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_2_640_s_206	9925594	Since very high soluble expression of rHbs always required a >2.5-fold molar excess of heme, this excess may be required for sufficient diffusion across the cell membrane to maintain an intracellular heme concentration high enough to drive the bimolecular reaction of heme with globin.	transcription
56893	1	335765	5	NULL	NULL	0	NULL	CO2			bind		covalently			Hb alpha-globin chains			amino terminus		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_22_16738_s_233	10747928	For example, the covalent binding of CO2 to the amino terminus of Hb alpha-globin chains lowers O2 affinity, and accordingly, O2 binding at the hemes triggers the dissociation of CO2 (the Haldane effect) ( 58).	transcription
56894	2	335765	5	NULL	NULL	0	NULL	statement 1			lowers					O2		affinity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_22_16738_s_233	10747928	For example, the covalent binding of CO2 to the amino terminus of Hb alpha-globin chains lowers O2 affinity, and accordingly, O2 binding at the hemes triggers the dissociation of CO2 (the Haldane effect) ( 58).	transcription
56895	3	335765	5	NULL	NULL	0	NULL	O2			bind					heme					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_22_16738_s_233	10747928	For example, the covalent binding of CO2 to the amino terminus of Hb alpha-globin chains lowers O2 affinity, and accordingly, O2 binding at the hemes triggers the dissociation of CO2 (the Haldane effect) ( 58).	transcription
56896	4	335765	5	NULL	NULL	0	NULL	statement 3			triggers					CO2		dissociation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_22_16738_s_233	10747928	For example, the covalent binding of CO2 to the amino terminus of Hb alpha-globin chains lowers O2 affinity, and accordingly, O2 binding at the hemes triggers the dissociation of CO2 (the Haldane effect) ( 58).	transcription
79067	1	335765	6	NULL	NULL	0	NULL	CO2	Chemical		bind					Hb alpha-globin			amino terminus		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_22_16738_s_233	10747928	For example, the covalent binding of CO2 to the amino terminus of Hb alpha-globin chains lowers O2 affinity, and accordingly, O2 binding at the hemes triggers the dissociation of CO2 (the Haldane effect) ( 58).	transcription
79068	2	335765	6	NULL	NULL	0	NULL	O2	Chemical		bind					heme	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_22_16738_s_233	10747928	For example, the covalent binding of CO2 to the amino terminus of Hb alpha-globin chains lowers O2 affinity, and accordingly, O2 binding at the hemes triggers the dissociation of CO2 (the Haldane effect) ( 58).	transcription
57886	1	335766	5	NULL	NULL	0	NULL	Ngb			coordinates to			proximal histidine residue		heme					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_39_36377_s_22	11473111	Nevertheless, according to multiple sequence alignment, key amino acid residues that are required for the function of these proteins and are conserved among a great variety of globins are present in the primary amino acid sequence of Ngb: namely a proximal histidine residue that coordinates to the heme (helical position F8), a distal histidine residue that might be involved in interactions with heme-bound ligands (E7), and a phenylalanine residue at CD1 that is involved in pi-pi interactions with the heme ( 4).	transcription
57887	2	335766	5	NULL	NULL	0	NULL	Ngb			is involved in		might be	distal histidine residue		heme-bound ligands		interaction with			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_39_36377_s_22	11473111	Nevertheless, according to multiple sequence alignment, key amino acid residues that are required for the function of these proteins and are conserved among a great variety of globins are present in the primary amino acid sequence of Ngb: namely a proximal histidine residue that coordinates to the heme (helical position F8), a distal histidine residue that might be involved in interactions with heme-bound ligands (E7), and a phenylalanine residue at CD1 that is involved in pi-pi interactions with the heme ( 4).	transcription
57888	3	335766	5	NULL	NULL	0	NULL	Ngb			is involved in			phenylalanine residue at CD1		heme		pi-pi interactions with			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_39_36377_s_22	11473111	Nevertheless, according to multiple sequence alignment, key amino acid residues that are required for the function of these proteins and are conserved among a great variety of globins are present in the primary amino acid sequence of Ngb: namely a proximal histidine residue that coordinates to the heme (helical position F8), a distal histidine residue that might be involved in interactions with heme-bound ligands (E7), and a phenylalanine residue at CD1 that is involved in pi-pi interactions with the heme ( 4).	transcription
57889	1	335768	5	NULL	NULL	0	NULL	K562 cells			is a type of					human erythroleukemia cells					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_7	14660636	The heme-dependent expression of beta-globin is a transcriptional event since the expression of the human beta-globin gene promoter-reporter gene containing the microlocus control region (muLCR) was inhibited when human erythroleukemia K562 cells and MEL cells were cultured with SA.	transcription
57890	2	335768	5	NULL	NULL	0	NULL	K562 cells			is cultured with					SA					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_7	14660636	The heme-dependent expression of beta-globin is a transcriptional event since the expression of the human beta-globin gene promoter-reporter gene containing the microlocus control region (muLCR) was inhibited when human erythroleukemia K562 cells and MEL cells were cultured with SA.	transcription
57891	3	335768	5	NULL	NULL	0	NULL	MEL cells			is cultured with					SA					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_7	14660636	The heme-dependent expression of beta-globin is a transcriptional event since the expression of the human beta-globin gene promoter-reporter gene containing the microlocus control region (muLCR) was inhibited when human erythroleukemia K562 cells and MEL cells were cultured with SA.	transcription
57892	4	335768	5	NULL	NULL	0	NULL	beta-globin gene promoter-reporter gene		human	contains									muLCR	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_7	14660636	The heme-dependent expression of beta-globin is a transcriptional event since the expression of the human beta-globin gene promoter-reporter gene containing the microlocus control region (muLCR) was inhibited when human erythroleukemia K562 cells and MEL cells were cultured with SA.	transcription
57893	5	335768	5	NULL	NULL	0	NULL	muLCR			is					microlocus control region					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_7	14660636	The heme-dependent expression of beta-globin is a transcriptional event since the expression of the human beta-globin gene promoter-reporter gene containing the microlocus control region (muLCR) was inhibited when human erythroleukemia K562 cells and MEL cells were cultured with SA.	transcription
57894	6	335768	5	NULL	NULL	0	NULL	statement 2			inhibits					statement 4					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_7	14660636	The heme-dependent expression of beta-globin is a transcriptional event since the expression of the human beta-globin gene promoter-reporter gene containing the microlocus control region (muLCR) was inhibited when human erythroleukemia K562 cells and MEL cells were cultured with SA.	transcription
57895	7	335768	5	NULL	NULL	0	NULL	statement 3			inhibits					statement 4					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_7	14660636	The heme-dependent expression of beta-globin is a transcriptional event since the expression of the human beta-globin gene promoter-reporter gene containing the microlocus control region (muLCR) was inhibited when human erythroleukemia K562 cells and MEL cells were cultured with SA.	transcription
57896	8	335768	5	NULL	NULL	0	NULL	beta-globin		expression of	is dependent on					heme					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_7	14660636	The heme-dependent expression of beta-globin is a transcriptional event since the expression of the human beta-globin gene promoter-reporter gene containing the microlocus control region (muLCR) was inhibited when human erythroleukemia K562 cells and MEL cells were cultured with SA.	transcription
57897	1	335770	5	NULL	NULL	0	NULL	globin			interacts with					heme					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_312_1_65_s_18	14630020	By means of various optical methods (ORD, CD, MORD) the interaction of globin with  heme was analysed to understand the specific function of hemoproteins such as reversible  oxygen binding (hemoglobin), splitting of hydrogen peroxide (catalase), and electron  transfer (cytochrome  c).	transcription
57898	2	335770	5	NULL	NULL	0	NULL	hemoglobin			is a type of					hemoproteins					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_312_1_65_s_18	14630020	By means of various optical methods (ORD, CD, MORD) the interaction of globin with  heme was analysed to understand the specific function of hemoproteins such as reversible  oxygen binding (hemoglobin), splitting of hydrogen peroxide (catalase), and electron  transfer (cytochrome  c).	transcription
57899	3	335770	5	NULL	NULL	0	NULL	catalase			is a type of					hemoproteins					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_312_1_65_s_18	14630020	By means of various optical methods (ORD, CD, MORD) the interaction of globin with  heme was analysed to understand the specific function of hemoproteins such as reversible  oxygen binding (hemoglobin), splitting of hydrogen peroxide (catalase), and electron  transfer (cytochrome  c).	transcription
57900	4	335770	5	NULL	NULL	0	NULL	cytochrome c			is a type of					hemoproteins					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_312_1_65_s_18	14630020	By means of various optical methods (ORD, CD, MORD) the interaction of globin with  heme was analysed to understand the specific function of hemoproteins such as reversible  oxygen binding (hemoglobin), splitting of hydrogen peroxide (catalase), and electron  transfer (cytochrome  c).	transcription
57901	5	335770	5	NULL	NULL	0	NULL	hemoglobin			bind		reversibly			oxygen					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_312_1_65_s_18	14630020	By means of various optical methods (ORD, CD, MORD) the interaction of globin with  heme was analysed to understand the specific function of hemoproteins such as reversible  oxygen binding (hemoglobin), splitting of hydrogen peroxide (catalase), and electron  transfer (cytochrome  c).	transcription
57902	6	335770	5	NULL	NULL	0	NULL	catalase			splits					hydrogen peroxide					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_312_1_65_s_18	14630020	By means of various optical methods (ORD, CD, MORD) the interaction of globin with  heme was analysed to understand the specific function of hemoproteins such as reversible  oxygen binding (hemoglobin), splitting of hydrogen peroxide (catalase), and electron  transfer (cytochrome  c).	transcription
57903	7	335770	5	NULL	NULL	0	NULL	cytochrome c			is involved in					electron transfer					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_312_1_65_s_18	14630020	By means of various optical methods (ORD, CD, MORD) the interaction of globin with  heme was analysed to understand the specific function of hemoproteins such as reversible  oxygen binding (hemoglobin), splitting of hydrogen peroxide (catalase), and electron  transfer (cytochrome  c).	transcription
57904	1	335771	5	NULL	NULL	0	NULL	GATA-1			bind		specifically			GSTP1-1				promoter	NULL		NULL	NULL	NULL	NULL	gw70_biochmbiophyrescomm_311_4_815_s_115	14623254	Specific GATA-1 binding to the GSTP1-1 promoter is  shown here by EMSA competition and supershift experiments as it was previously described  for erythroid-specific genes such as globin [  42] and genes involved in heme biosynthesis [  43].	transcription
79069	1	335771	6	NULL	NULL	0	NULL	GATA-1	GP		bind					GSTP1-1 	GP			promoter	NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_311_4_815_s_115	14623254	Specific GATA-1 binding to the GSTP1-1 promoter is  shown here by EMSA competition and supershift experiments as it was previously described  for erythroid-specific genes such as globin [  42] and genes involved in heme biosynthesis [  43].	transcription
57905	1	335772	5	NULL	NULL	0	NULL	heme			bind		directly			Bach1					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_16_5857_s_16	12897155	Notably, heme directly binds to and inhibits the mammalian transcriptional repressor Bach1 ( ), a dimerization partner of the Maf family proteins, which controls the expression of a wide array of genes, including oxidative stress-responsive genes and globin genes ( ,  - ,  ,  ,  ).	transcription
57906	2	335772	5	NULL	NULL	0	NULL	statement 1			inhibits					Bach1					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_16_5857_s_16	12897155	Notably, heme directly binds to and inhibits the mammalian transcriptional repressor Bach1 ( ), a dimerization partner of the Maf family proteins, which controls the expression of a wide array of genes, including oxidative stress-responsive genes and globin genes ( ,  - ,  ,  ,  ).	transcription
57907	3	335772	5	NULL	NULL	0	NULL	Bach1			is a type of					mammalian transcriptional repressor					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_16_5857_s_16	12897155	Notably, heme directly binds to and inhibits the mammalian transcriptional repressor Bach1 ( ), a dimerization partner of the Maf family proteins, which controls the expression of a wide array of genes, including oxidative stress-responsive genes and globin genes ( ,  - ,  ,  ,  ).	transcription
57908	4	335772	5	NULL	NULL	0	NULL	Bach1			is a dimerization partner of					Maf family proteins					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_16_5857_s_16	12897155	Notably, heme directly binds to and inhibits the mammalian transcriptional repressor Bach1 ( ), a dimerization partner of the Maf family proteins, which controls the expression of a wide array of genes, including oxidative stress-responsive genes and globin genes ( ,  - ,  ,  ,  ).	transcription
57909	1	335774	5	NULL	NULL	0	NULL	alpha-globin chain			assemble into					hemoglobin					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_6778_s_15	14672943	A deficiency of heme, which is required for the assembly of alpha- and beta-globin chains into hemoglobin, induces the activation of HRI, which subsequently phosphorylates the alpha-subunit of eIF2, leading to the inhibition of polypeptide chain initiation and the arrest of protein synthesis.	transcription
57910	2	335774	5	NULL	NULL	0	NULL	beta-globin chain			assemble into					hemoglobin					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_6778_s_15	14672943	A deficiency of heme, which is required for the assembly of alpha- and beta-globin chains into hemoglobin, induces the activation of HRI, which subsequently phosphorylates the alpha-subunit of eIF2, leading to the inhibition of polypeptide chain initiation and the arrest of protein synthesis.	transcription
57911	3	335774	5	NULL	NULL	0	NULL	heme			is required for					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_6778_s_15	14672943	A deficiency of heme, which is required for the assembly of alpha- and beta-globin chains into hemoglobin, induces the activation of HRI, which subsequently phosphorylates the alpha-subunit of eIF2, leading to the inhibition of polypeptide chain initiation and the arrest of protein synthesis.	transcription
57912	4	335774	5	NULL	NULL	0	NULL	heme			is required for					statement 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_6778_s_15	14672943	A deficiency of heme, which is required for the assembly of alpha- and beta-globin chains into hemoglobin, induces the activation of HRI, which subsequently phosphorylates the alpha-subunit of eIF2, leading to the inhibition of polypeptide chain initiation and the arrest of protein synthesis.	transcription
57913	5	335774	5	NULL	NULL	0	NULL	heme		deficiency of	induces					HRI		activation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_6778_s_15	14672943	A deficiency of heme, which is required for the assembly of alpha- and beta-globin chains into hemoglobin, induces the activation of HRI, which subsequently phosphorylates the alpha-subunit of eIF2, leading to the inhibition of polypeptide chain initiation and the arrest of protein synthesis.	transcription
57914	6	335774	5	NULL	NULL	0	NULL	HRI		activated	phosphorylates		subsequently			eIF2			alpha-subunit		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_6778_s_15	14672943	A deficiency of heme, which is required for the assembly of alpha- and beta-globin chains into hemoglobin, induces the activation of HRI, which subsequently phosphorylates the alpha-subunit of eIF2, leading to the inhibition of polypeptide chain initiation and the arrest of protein synthesis.	transcription
57915	7	335774	5	NULL	NULL	0	NULL	statement 6			inhibits					polypeptide chain		initiation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_6778_s_15	14672943	A deficiency of heme, which is required for the assembly of alpha- and beta-globin chains into hemoglobin, induces the activation of HRI, which subsequently phosphorylates the alpha-subunit of eIF2, leading to the inhibition of polypeptide chain initiation and the arrest of protein synthesis.	transcription
57916	8	335774	5	NULL	NULL	0	NULL	statement 7			arrests					protein		synthesis of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_6778_s_15	14672943	A deficiency of heme, which is required for the assembly of alpha- and beta-globin chains into hemoglobin, induces the activation of HRI, which subsequently phosphorylates the alpha-subunit of eIF2, leading to the inhibition of polypeptide chain initiation and the arrest of protein synthesis.	transcription
79072	1	335774	6	NULL	NULL	0	NULL	heme	GP	deficiency of	induces					HRI	GP	activation of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_6778_s_15	14672943	A deficiency of heme, which is required for the assembly of alpha- and beta-globin chains into hemoglobin, induces the activation of HRI, which subsequently phosphorylates the alpha-subunit of eIF2, leading to the inhibition of polypeptide chain initiation and the arrest of protein synthesis.	transcription
57917	1	335775	5	NULL	NULL	0	NULL	Bach1		endogenous	bind					DNA					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_148	14660636	We then conducted a conventional gel-shift assay using a synthetic oligonucleotide probe containing a MARE from the chicken beta-globin 3' enhancer to examine whether the DNA binding activity of endogenous Bach1 is indeed regulated by heme.	transcription
57918	2	335775	5	NULL	NULL	0	NULL	heme			regulates		potentially			statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_7_5480_s_148	14660636	We then conducted a conventional gel-shift assay using a synthetic oligonucleotide probe containing a MARE from the chicken beta-globin 3' enhancer to examine whether the DNA binding activity of endogenous Bach1 is indeed regulated by heme.	transcription
58416	1	335777	5	NULL	NULL	0	NULL	H93G (+Imd)		mutant	mimics					Mb		NT			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24637_s_236	16774917	The H93G (+Imd) mutant serves as a mimic of NT Mb in which the covalent bond between heme and globin is cleaved and an exogenous imidazole binds to iron freely in the proximal cavity ( ).	transcription
58417	2	335777	5	NULL	NULL	0	NULL	heme			bind		covalently			globin					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_34_24637_s_236	16774917	The H93G (+Imd) mutant serves as a mimic of NT Mb in which the covalent bond between heme and globin is cleaved and an exogenous imidazole binds to iron freely in the proximal cavity ( ).	transcription
58418	3	335777	5	NULL	NULL	0	NULL	statement 2			occurs in					Mb		NT			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24637_s_236	16774917	The H93G (+Imd) mutant serves as a mimic of NT Mb in which the covalent bond between heme and globin is cleaved and an exogenous imidazole binds to iron freely in the proximal cavity ( ).	transcription
58419	4	335777	5	NULL	NULL	0	NULL	statement 2			undergoes					cleavage					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_34_24637_s_236	16774917	The H93G (+Imd) mutant serves as a mimic of NT Mb in which the covalent bond between heme and globin is cleaved and an exogenous imidazole binds to iron freely in the proximal cavity ( ).	transcription
58420	5	335777	5	NULL	NULL	0	NULL	imidazole		exogenous	bind		freely			iron					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_34_24637_s_236	16774917	The H93G (+Imd) mutant serves as a mimic of NT Mb in which the covalent bond between heme and globin is cleaved and an exogenous imidazole binds to iron freely in the proximal cavity ( ).	transcription
58421	6	335777	5	NULL	NULL	0	NULL	statement 5			occurs in					Mb		NT	proximal cavity		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_34_24637_s_236	16774917	The H93G (+Imd) mutant serves as a mimic of NT Mb in which the covalent bond between heme and globin is cleaved and an exogenous imidazole binds to iron freely in the proximal cavity ( ).	transcription
58422	7	335777	5	NULL	NULL	0	NULL	statement 4			leads to					statement 5					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_34_24637_s_236	16774917	The H93G (+Imd) mutant serves as a mimic of NT Mb in which the covalent bond between heme and globin is cleaved and an exogenous imidazole binds to iron freely in the proximal cavity ( ).	transcription
79073	1	335777	6	NULL	NULL	0	NULL	imidazole	Chemical		bind					iron	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_34_24637_s_236	16774917	The H93G (+Imd) mutant serves as a mimic of NT Mb in which the covalent bond between heme and globin is cleaved and an exogenous imidazole binds to iron freely in the proximal cavity ( ).	transcription
58424	1	335779	5	NULL	NULL	0	NULL	ApPgb		Archaea Aeropyrum pernix	bind					O2					NULL		0	NULL	NULL	NULL	gw70_pnas_101_17_6675_s_16	15096613	Here, we show that two proteins  ApPgb and  MaPgb, identified from the  Archaea Aeropyrum pernix and  Methanosarcina acetivorans, respectively, conform to the globin sequence motifs, contain heme, and demonstrably bind O2, CO, and NO.	transcription
58425	2	335779	5	NULL	NULL	0	NULL	ApPgb		Archaea Aeropyrum pernix	bind					CO					NULL		0	NULL	NULL	NULL	gw70_pnas_101_17_6675_s_16	15096613	Here, we show that two proteins  ApPgb and  MaPgb, identified from the  Archaea Aeropyrum pernix and  Methanosarcina acetivorans, respectively, conform to the globin sequence motifs, contain heme, and demonstrably bind O2, CO, and NO.	transcription
58426	3	335779	5	NULL	NULL	0	NULL	ApPgb		Archaea Aeropyrum pernix	bind					NO					NULL		0	NULL	NULL	NULL	gw70_pnas_101_17_6675_s_16	15096613	Here, we show that two proteins  ApPgb and  MaPgb, identified from the  Archaea Aeropyrum pernix and  Methanosarcina acetivorans, respectively, conform to the globin sequence motifs, contain heme, and demonstrably bind O2, CO, and NO.	transcription
58427	4	335779	5	NULL	NULL	0	NULL	MaPgb		Methanosarcina acetivorans	bind					O2					NULL		0	NULL	NULL	NULL	gw70_pnas_101_17_6675_s_16	15096613	Here, we show that two proteins  ApPgb and  MaPgb, identified from the  Archaea Aeropyrum pernix and  Methanosarcina acetivorans, respectively, conform to the globin sequence motifs, contain heme, and demonstrably bind O2, CO, and NO.	transcription
58428	5	335779	5	NULL	NULL	0	NULL	MaPgb		Methanosarcina acetivorans	bind					CO					NULL		0	NULL	NULL	NULL	gw70_pnas_101_17_6675_s_16	15096613	Here, we show that two proteins  ApPgb and  MaPgb, identified from the  Archaea Aeropyrum pernix and  Methanosarcina acetivorans, respectively, conform to the globin sequence motifs, contain heme, and demonstrably bind O2, CO, and NO.	transcription
58429	6	335779	5	NULL	NULL	0	NULL	MaPgb		Methanosarcina acetivorans	bind					NO					NULL		0	NULL	NULL	NULL	gw70_pnas_101_17_6675_s_16	15096613	Here, we show that two proteins  ApPgb and  MaPgb, identified from the  Archaea Aeropyrum pernix and  Methanosarcina acetivorans, respectively, conform to the globin sequence motifs, contain heme, and demonstrably bind O2, CO, and NO.	transcription
79074	1	335779	6	NULL	NULL	0	NULL	ApPgb	GP		bind					O2	Chemical				NULL		0	NULL	NULL	NULL	gw70_pnas_101_17_6675_s_16	15096613	Here, we show that two proteins  ApPgb and  MaPgb, identified from the  Archaea Aeropyrum pernix and  Methanosarcina acetivorans, respectively, conform to the globin sequence motifs, contain heme, and demonstrably bind O2, CO, and NO.	transcription
79075	2	335779	6	NULL	NULL	0	NULL	ApPgb	GP		bind					CO	Chemical				NULL		0	NULL	NULL	NULL	gw70_pnas_101_17_6675_s_16	15096613	Here, we show that two proteins  ApPgb and  MaPgb, identified from the  Archaea Aeropyrum pernix and  Methanosarcina acetivorans, respectively, conform to the globin sequence motifs, contain heme, and demonstrably bind O2, CO, and NO.	transcription
79076	3	335779	6	NULL	NULL	0	NULL	ApPgb	Chemical		bind					NO	Chemical				NULL		0	NULL	NULL	NULL	gw70_pnas_101_17_6675_s_16	15096613	Here, we show that two proteins  ApPgb and  MaPgb, identified from the  Archaea Aeropyrum pernix and  Methanosarcina acetivorans, respectively, conform to the globin sequence motifs, contain heme, and demonstrably bind O2, CO, and NO.	transcription
79077	4	335779	6	NULL	NULL	0	NULL	MaPgb	GP		bind					O2	Chemical				NULL		0	NULL	NULL	NULL	gw70_pnas_101_17_6675_s_16	15096613	Here, we show that two proteins  ApPgb and  MaPgb, identified from the  Archaea Aeropyrum pernix and  Methanosarcina acetivorans, respectively, conform to the globin sequence motifs, contain heme, and demonstrably bind O2, CO, and NO.	transcription
79078	5	335779	6	NULL	NULL	0	NULL	MaPgb	GP		bind					CO	Chemical				NULL		0	NULL	NULL	NULL	gw70_pnas_101_17_6675_s_16	15096613	Here, we show that two proteins  ApPgb and  MaPgb, identified from the  Archaea Aeropyrum pernix and  Methanosarcina acetivorans, respectively, conform to the globin sequence motifs, contain heme, and demonstrably bind O2, CO, and NO.	transcription
79079	6	335779	6	NULL	NULL	0	NULL	MaPgb	GP		bind					NO	Chemical				NULL		0	NULL	NULL	NULL	gw70_pnas_101_17_6675_s_16	15096613	Here, we show that two proteins  ApPgb and  MaPgb, identified from the  Archaea Aeropyrum pernix and  Methanosarcina acetivorans, respectively, conform to the globin sequence motifs, contain heme, and demonstrably bind O2, CO, and NO.	transcription
58430	1	335780	5	NULL	NULL	0	NULL	HemAT- Hs			bind		reversibly			O2					NULL		0	NULL	NULL	NULL	gw70_pnas_101_17_6675_s_96	15096613	The archaeal Pgbs,  ApPgb and  MaPgb, were exactly 195 aa long: the minimum length found to be required for heme and reversible O2 binding by the globin-coupled aerotaxis transducer HemAT- Hs (9 ).	transcription
58431	2	335780	5	NULL	NULL	0	NULL	HemAT- Hs			is coupled to					globin					NULL		0	NULL	NULL	NULL	gw70_pnas_101_17_6675_s_96	15096613	The archaeal Pgbs,  ApPgb and  MaPgb, were exactly 195 aa long: the minimum length found to be required for heme and reversible O2 binding by the globin-coupled aerotaxis transducer HemAT- Hs (9 ).	transcription
58432	3	335780	5	NULL	NULL	0	NULL	HemAT- Hs			is a type of					aerotaxis transducer					NULL		0	NULL	NULL	NULL	gw70_pnas_101_17_6675_s_96	15096613	The archaeal Pgbs,  ApPgb and  MaPgb, were exactly 195 aa long: the minimum length found to be required for heme and reversible O2 binding by the globin-coupled aerotaxis transducer HemAT- Hs (9 ).	transcription
58433	1	335781	5	NULL	NULL	0	NULL	heme		intracellular levels of	regulates					Maf protein partners		exchange of;;small			NULL		0	NULL	NULL	NULL	gw70_pnas_101_6_1461_s_215	14747657	Our results suggest that intracellular levels of heme regulate the exchange of small Maf protein partners in not only the stress-responsive control of HO-1 but also the differentiation-associated control of beta-globin expression.	transcription
58434	2	335781	5	NULL	NULL	0	NULL	statement 1			occurs in					HO-1		stress-responsive control of			NULL		0	NULL	NULL	NULL	gw70_pnas_101_6_1461_s_215	14747657	Our results suggest that intracellular levels of heme regulate the exchange of small Maf protein partners in not only the stress-responsive control of HO-1 but also the differentiation-associated control of beta-globin expression.	transcription
58435	3	335781	5	NULL	NULL	0	NULL	statement 1			occurs in					beta-globin		differentiation-associated control of;;expression of			NULL		0	NULL	NULL	NULL	gw70_pnas_101_6_1461_s_215	14747657	Our results suggest that intracellular levels of heme regulate the exchange of small Maf protein partners in not only the stress-responsive control of HO-1 but also the differentiation-associated control of beta-globin expression.	transcription
58436	1	335782	5	NULL	NULL	0	NULL	N. meningitidis			bind					hemoglobin		biotinylated			NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_162_2_227_s_96	9627957	The results are consistent with other studies which show that the binding of  N. meningitidis to biotinylated hemoglobin is inhibited by unlabeled hemoglobin but not heme, suggesting that the hemoglobin binding protein of  N. meningitidis recognizes the globin moiety of hemoglobin  [ 18].	transcription
58437	2	335782	5	NULL	NULL	0	NULL	hemoglobin		unlabeled	inhibits					statement 1					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_162_2_227_s_96	9627957	The results are consistent with other studies which show that the binding of  N. meningitidis to biotinylated hemoglobin is inhibited by unlabeled hemoglobin but not heme, suggesting that the hemoglobin binding protein of  N. meningitidis recognizes the globin moiety of hemoglobin  [ 18].	transcription
58438	3	335782	5	NULL	NULL	0	NULL	heme			does not inhibit					statement 1					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_162_2_227_s_96	9627957	The results are consistent with other studies which show that the binding of  N. meningitidis to biotinylated hemoglobin is inhibited by unlabeled hemoglobin but not heme, suggesting that the hemoglobin binding protein of  N. meningitidis recognizes the globin moiety of hemoglobin  [ 18].	transcription
58439	4	335782	5	NULL	NULL	0	NULL	hemoglobin binding protein		N. meningitidis	recognizes					hemoglobin			globin moiety		NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_162_2_227_s_96	9627957	The results are consistent with other studies which show that the binding of  N. meningitidis to biotinylated hemoglobin is inhibited by unlabeled hemoglobin but not heme, suggesting that the hemoglobin binding protein of  N. meningitidis recognizes the globin moiety of hemoglobin  [ 18].	transcription
58440	5	335782	5	NULL	NULL	0	NULL	statement 2			suggest					statement 4					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_162_2_227_s_96	9627957	The results are consistent with other studies which show that the binding of  N. meningitidis to biotinylated hemoglobin is inhibited by unlabeled hemoglobin but not heme, suggesting that the hemoglobin binding protein of  N. meningitidis recognizes the globin moiety of hemoglobin  [ 18].	transcription
58441	6	335782	5	NULL	NULL	0	NULL	statement 3			suggest					statement 4					NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_162_2_227_s_96	9627957	The results are consistent with other studies which show that the binding of  N. meningitidis to biotinylated hemoglobin is inhibited by unlabeled hemoglobin but not heme, suggesting that the hemoglobin binding protein of  N. meningitidis recognizes the globin moiety of hemoglobin  [ 18].	transcription
79080	1	335782	6	NULL	NULL	0	NULL	N. meningitidis	Organism		bind					hemoglobin	GP	bioytinylated			NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_162_2_227_s_96	9627957	The results are consistent with other studies which show that the binding of  N. meningitidis to biotinylated hemoglobin is inhibited by unlabeled hemoglobin but not heme, suggesting that the hemoglobin binding protein of  N. meningitidis recognizes the globin moiety of hemoglobin  [ 18].	transcription
58442	1	335783	5	NULL	NULL	0	NULL	NF-E2			bind									TGCTGA(G/C)TCA	NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_14_10715_s_12	11154691	NF-E2 binds to an extended AP-1-like element, TGCTGA(G/C)TCA, which is found in the locus control regions (LCRs) of the alpha- and beta-globin genes and in the promoters of several heme biosynthetic enzyme genes (for review see Refs.	transcription
58443	2	335783	5	NULL	NULL	0	NULL	TGCTGA(G/C)TCA			is					AP-1-like element					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_14_10715_s_12	11154691	NF-E2 binds to an extended AP-1-like element, TGCTGA(G/C)TCA, which is found in the locus control regions (LCRs) of the alpha- and beta-globin genes and in the promoters of several heme biosynthetic enzyme genes (for review see Refs.	transcription
58444	3	335783	5	NULL	NULL	0	NULL	AP-1-like element			is located in					alpha-globin gene				LCRs	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_14_10715_s_12	11154691	NF-E2 binds to an extended AP-1-like element, TGCTGA(G/C)TCA, which is found in the locus control regions (LCRs) of the alpha- and beta-globin genes and in the promoters of several heme biosynthetic enzyme genes (for review see Refs.	transcription
58445	4	335783	5	NULL	NULL	0	NULL	AP-1-like element			is located in					beta-globin gene				LCRs	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_14_10715_s_12	11154691	NF-E2 binds to an extended AP-1-like element, TGCTGA(G/C)TCA, which is found in the locus control regions (LCRs) of the alpha- and beta-globin genes and in the promoters of several heme biosynthetic enzyme genes (for review see Refs.	transcription
79081	1	335783	6	NULL	NULL	0	NULL	NF-E2	GP		bind									AP-1-like element	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_14_10715_s_12	11154691	NF-E2 binds to an extended AP-1-like element, TGCTGA(G/C)TCA, which is found in the locus control regions (LCRs) of the alpha- and beta-globin genes and in the promoters of several heme biosynthetic enzyme genes (for review see Refs.	transcription
58446	1	335784	5	NULL	NULL	0	NULL	globin		Vitreoscilla	contains		only						heme protein domain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_46_35868_s_239	10915782	Interestingly, the well studied globin from  Vitreoscilla, which contains only a heme protein domain and no bound flavin, is a homodimer and the ferric protein displays anticooperative ligand binding behavior in solution ( 57).	transcription
58447	2	335784	5	NULL	NULL	0	NULL	globin		Vitreoscilla	does not bind					flavin					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_46_35868_s_239	10915782	Interestingly, the well studied globin from  Vitreoscilla, which contains only a heme protein domain and no bound flavin, is a homodimer and the ferric protein displays anticooperative ligand binding behavior in solution ( 57).	transcription
58448	3	335784	5	NULL	NULL	0	NULL	globin		Vitreoscilla	forms					homodimer					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_46_35868_s_239	10915782	Interestingly, the well studied globin from  Vitreoscilla, which contains only a heme protein domain and no bound flavin, is a homodimer and the ferric protein displays anticooperative ligand binding behavior in solution ( 57).	transcription
58449	4	335784	5	NULL	NULL	0	NULL	ferric protein			bind					ligand		anticooperative			NULL	solution	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_46_35868_s_239	10915782	Interestingly, the well studied globin from  Vitreoscilla, which contains only a heme protein domain and no bound flavin, is a homodimer and the ferric protein displays anticooperative ligand binding behavior in solution ( 57).	transcription
58450	1	335785	5	NULL	NULL	0	NULL	globin		structure of	controls					hemoglobins		redox potential of	heme site		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_50_39048_s_10	10984477	The globin structure controls the redox potential of the heme site of hemoglobins (Hbs)1 and myoglobins (Mbs), protects them from rapid oxidation, and thereby allows for reversible oxygen binding.	transcription
58451	2	335785	5	NULL	NULL	0	NULL	globin		structure of	controls					myoglobins		redox potential of	heme site		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_50_39048_s_10	10984477	The globin structure controls the redox potential of the heme site of hemoglobins (Hbs)1 and myoglobins (Mbs), protects them from rapid oxidation, and thereby allows for reversible oxygen binding.	transcription
58452	3	335785	5	NULL	NULL	0	NULL	globin		structure of	protects					hemoglobins		rapid oxidation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_50_39048_s_10	10984477	The globin structure controls the redox potential of the heme site of hemoglobins (Hbs)1 and myoglobins (Mbs), protects them from rapid oxidation, and thereby allows for reversible oxygen binding.	transcription
58453	4	335785	5	NULL	NULL	0	NULL	statement 3			allows					oxygen		reversible binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_50_39048_s_10	10984477	The globin structure controls the redox potential of the heme site of hemoglobins (Hbs)1 and myoglobins (Mbs), protects them from rapid oxidation, and thereby allows for reversible oxygen binding.	transcription
58454	5	335785	5	NULL	NULL	0	NULL	globin		structure of	protects					myoglobins		rapid oxidation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_50_39048_s_10	10984477	The globin structure controls the redox potential of the heme site of hemoglobins (Hbs)1 and myoglobins (Mbs), protects them from rapid oxidation, and thereby allows for reversible oxygen binding.	transcription
58455	6	335785	5	NULL	NULL	0	NULL	statement 5			allows					oxygen		reversible binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_50_39048_s_10	10984477	The globin structure controls the redox potential of the heme site of hemoglobins (Hbs)1 and myoglobins (Mbs), protects them from rapid oxidation, and thereby allows for reversible oxygen binding.	transcription
79082	1	335785	6	NULL	NULL	0	NULL	hemoglobin	GP		bind					oxygen	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_50_39048_s_10	10984477	The globin structure controls the redox potential of the heme site of hemoglobins (Hbs)1 and myoglobins (Mbs), protects them from rapid oxidation, and thereby allows for reversible oxygen binding.	transcription
79083	2	335785	6	NULL	NULL	0	NULL	myoglobin	GP		bind					oxygen	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_50_39048_s_10	10984477	The globin structure controls the redox potential of the heme site of hemoglobins (Hbs)1 and myoglobins (Mbs), protects them from rapid oxidation, and thereby allows for reversible oxygen binding.	transcription
58456	1	335786	5	NULL	NULL	0	NULL	EKLF protein			decrease during					erythroid		terminal differentiation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_37_23793_s_181	9726989	Although EKLF protein decreased during erythroid terminal differentiation, down-regulation of EKLF by the antisense construct prior to induction by epo severely inhibited transcription of globin and heme enzyme genes.	transcription
58457	2	335786	5	NULL	NULL	0	NULL	EKLF		down-regulation of	inhibit		severely			globin gene		transcription of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_37_23793_s_181	9726989	Although EKLF protein decreased during erythroid terminal differentiation, down-regulation of EKLF by the antisense construct prior to induction by epo severely inhibited transcription of globin and heme enzyme genes.	transcription
58458	3	335786	5	NULL	NULL	0	NULL	EKLF		down-regulation of	inhibit		severely			heme enzyme gene		transcription of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_37_23793_s_181	9726989	Although EKLF protein decreased during erythroid terminal differentiation, down-regulation of EKLF by the antisense construct prior to induction by epo severely inhibited transcription of globin and heme enzyme genes.	transcription
58459	4	335786	5	NULL	NULL	0	NULL	statement 2			occurs prior to					epo		induction by			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_37_23793_s_181	9726989	Although EKLF protein decreased during erythroid terminal differentiation, down-regulation of EKLF by the antisense construct prior to induction by epo severely inhibited transcription of globin and heme enzyme genes.	transcription
58460	5	335786	5	NULL	NULL	0	NULL	statement 3			occurs prior to					epo		induction by			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_37_23793_s_181	9726989	Although EKLF protein decreased during erythroid terminal differentiation, down-regulation of EKLF by the antisense construct prior to induction by epo severely inhibited transcription of globin and heme enzyme genes.	transcription
79084	1	335786	6	NULL	NULL	0	NULL	EKLF protein	GP		decreases during					erythroid terminal	cell	differentiation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_37_23793_s_181	9726989	Although EKLF protein decreased during erythroid terminal differentiation, down-regulation of EKLF by the antisense construct prior to induction by epo severely inhibited transcription of globin and heme enzyme genes.	transcription
58570	1	335787	5	NULL	NULL	0	NULL	cyanide ion			bind					heme Fe atom					NULL		0	NULL	NULL	NULL	gw60_pnas_100_10_5766_s_8	12719529	All 12 subunits display a cyanide ion bound to the heme Fe atom, stabilized by a tight hydrogen-bonded network based on the (globin very rare) TyrCD1 and TrpG8 residues.	transcription
79085	1	335787	6	NULL	NULL	0	NULL	cyanide ion	Chemical		bind					heme Fe atom	Chemical				NULL		0	NULL	NULL	NULL	gw60_pnas_100_10_5766_s_8	12719529	All 12 subunits display a cyanide ion bound to the heme Fe atom, stabilized by a tight hydrogen-bonded network based on the (globin very rare) TyrCD1 and TrpG8 residues.	transcription
58571	1	335789	5	NULL	NULL	0	NULL	iron chelation/DFO			inhibits					heme		biosynthesis of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_34_36048_s_181	15169765	To confirm that this differential expression pattern is HIF-derived, rather than from an iron chelation/DFO-mediated inhibition of heme biosynthesis, which, in turn, could lead to moderate down-regulation of fly globin transcription, it was necessary to look for similar responses in other HRE-flanked genes encoding heme-free products.	transcription
58572	2	335789	5	NULL	NULL	0	NULL	statement 1			down-regulates		moderately			globin		transcription of;;fly			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_34_36048_s_181	15169765	To confirm that this differential expression pattern is HIF-derived, rather than from an iron chelation/DFO-mediated inhibition of heme biosynthesis, which, in turn, could lead to moderate down-regulation of fly globin transcription, it was necessary to look for similar responses in other HRE-flanked genes encoding heme-free products.	transcription
58574	1	335790	5	NULL	NULL	0	NULL	HRI			bind			NTD		CO					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_99_s_146	12922173	The present study suggests that (1) the CO binding behavior of HRI-NTD is unusual for a globin-type heme protein, and (2) the CO molecule binds to the heme in HRI-NTD in an upright manner, forming weak interactions with nearby amino acids, according to the resonance Raman spectroscopy.	transcription
58575	2	335790	5	NULL	NULL	0	NULL	globin-type heme protein			does not bind					CO					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_99_s_146	12922173	The present study suggests that (1) the CO binding behavior of HRI-NTD is unusual for a globin-type heme protein, and (2) the CO molecule binds to the heme in HRI-NTD in an upright manner, forming weak interactions with nearby amino acids, according to the resonance Raman spectroscopy.	transcription
58576	3	335790	5	NULL	NULL	0	NULL	heme			is present in					HRI			NTD		NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_99_s_146	12922173	The present study suggests that (1) the CO binding behavior of HRI-NTD is unusual for a globin-type heme protein, and (2) the CO molecule binds to the heme in HRI-NTD in an upright manner, forming weak interactions with nearby amino acids, according to the resonance Raman spectroscopy.	transcription
58577	4	335790	5	NULL	NULL	0	NULL	CO			bind					statement 3					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_99_s_146	12922173	The present study suggests that (1) the CO binding behavior of HRI-NTD is unusual for a globin-type heme protein, and (2) the CO molecule binds to the heme in HRI-NTD in an upright manner, forming weak interactions with nearby amino acids, according to the resonance Raman spectroscopy.	transcription
79086	1	335790	6	NULL	NULL	0	NULL	CO	Chemical		bind					HRI	GP		NTD		NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_99_s_146	12922173	The present study suggests that (1) the CO binding behavior of HRI-NTD is unusual for a globin-type heme protein, and (2) the CO molecule binds to the heme in HRI-NTD in an upright manner, forming weak interactions with nearby amino acids, according to the resonance Raman spectroscopy.	transcription
79087	2	335790	6	NULL	NULL	0	NULL	CO	GP		bind					heme	GP		HRI-NTD		NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1650_1_99_s_146	12922173	The present study suggests that (1) the CO binding behavior of HRI-NTD is unusual for a globin-type heme protein, and (2) the CO molecule binds to the heme in HRI-NTD in an upright manner, forming weak interactions with nearby amino acids, according to the resonance Raman spectroscopy.	transcription
58578	1	335791	5	NULL	NULL	0	NULL	heme			stimulates					globin chains		expression of			NULL	erythroid cells	0	NULL	NULL	NULL	gw60_molcellbiol_18_7_3819_s_14	9632766	For example, heme stimulates the expression of globin chains in erythroid cells and cytochrome P-450 in hepatic cells ( 6,  9,  36), activates protein synthesis through the heme-regulated inhibitor kinase ( 7), and regulates the transport of numerous enzymes and the assembly of hemoglobin and cytochrome complexes ( 24,  31).	transcription
58579	2	335791	5	NULL	NULL	0	NULL	heme			stimulates					cytochrome P-450					NULL	hepatic cells 	0	NULL	NULL	NULL	gw60_molcellbiol_18_7_3819_s_14	9632766	For example, heme stimulates the expression of globin chains in erythroid cells and cytochrome P-450 in hepatic cells ( 6,  9,  36), activates protein synthesis through the heme-regulated inhibitor kinase ( 7), and regulates the transport of numerous enzymes and the assembly of hemoglobin and cytochrome complexes ( 24,  31).	transcription
58580	3	335791	5	NULL	NULL	0	NULL	inhibitor kinase			is regulated by					heme					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_7_3819_s_14	9632766	For example, heme stimulates the expression of globin chains in erythroid cells and cytochrome P-450 in hepatic cells ( 6,  9,  36), activates protein synthesis through the heme-regulated inhibitor kinase ( 7), and regulates the transport of numerous enzymes and the assembly of hemoglobin and cytochrome complexes ( 24,  31).	transcription
58581	4	335791	5	NULL	NULL	0	NULL	heme			activates					protein synthesis					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_7_3819_s_14	9632766	For example, heme stimulates the expression of globin chains in erythroid cells and cytochrome P-450 in hepatic cells ( 6,  9,  36), activates protein synthesis through the heme-regulated inhibitor kinase ( 7), and regulates the transport of numerous enzymes and the assembly of hemoglobin and cytochrome complexes ( 24,  31).	transcription
58582	5	335791	5	NULL	NULL	0	NULL	statement 4			occurs through					statement 3					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_7_3819_s_14	9632766	For example, heme stimulates the expression of globin chains in erythroid cells and cytochrome P-450 in hepatic cells ( 6,  9,  36), activates protein synthesis through the heme-regulated inhibitor kinase ( 7), and regulates the transport of numerous enzymes and the assembly of hemoglobin and cytochrome complexes ( 24,  31).	transcription
58583	6	335791	5	NULL	NULL	0	NULL	heme			regulates					hemoglobin		assembly of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_7_3819_s_14	9632766	For example, heme stimulates the expression of globin chains in erythroid cells and cytochrome P-450 in hepatic cells ( 6,  9,  36), activates protein synthesis through the heme-regulated inhibitor kinase ( 7), and regulates the transport of numerous enzymes and the assembly of hemoglobin and cytochrome complexes ( 24,  31).	transcription
58584	7	335791	5	NULL	NULL	0	NULL	heme			regulates					cytochrome complexes		assembly of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_7_3819_s_14	9632766	For example, heme stimulates the expression of globin chains in erythroid cells and cytochrome P-450 in hepatic cells ( 6,  9,  36), activates protein synthesis through the heme-regulated inhibitor kinase ( 7), and regulates the transport of numerous enzymes and the assembly of hemoglobin and cytochrome complexes ( 24,  31).	transcription
79088	1	335791	6	NULL	NULL	0	NULL	heme	GP		stimulates					hepatic cells	cell	expression of	globin chains		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_18_7_3819_s_14	9632766	For example, heme stimulates the expression of globin chains in erythroid cells and cytochrome P-450 in hepatic cells ( 6,  9,  36), activates protein synthesis through the heme-regulated inhibitor kinase ( 7), and regulates the transport of numerous enzymes and the assembly of hemoglobin and cytochrome complexes ( 24,  31).	transcription
79089	2	335791	6	NULL	NULL	0	NULL	heme	GP		stimulates					cytochrome P-450	GP	expression of			NULL	hepatic cells	0	NULL	NULL	NULL	gw60_molcellbiol_18_7_3819_s_14	9632766	For example, heme stimulates the expression of globin chains in erythroid cells and cytochrome P-450 in hepatic cells ( 6,  9,  36), activates protein synthesis through the heme-regulated inhibitor kinase ( 7), and regulates the transport of numerous enzymes and the assembly of hemoglobin and cytochrome complexes ( 24,  31).	transcription
58585	1	335792	5	NULL	NULL	0	NULL	alpha chains		nascent	interacts with					heme					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_16_13415_s_154	11827978	This indicates that nascent alpha chains having 86 amino acids possess a structure that allows interaction with heme or that heme binding to nascent globin chains promotes formation of the proper tertiary structure of the growing polypeptide chain on polyribosomes ( 19,  20).	transcription
58586	2	335792	5	NULL	NULL	0	NULL	heme			bind					globin chains		nascent			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_16_13415_s_154	11827978	This indicates that nascent alpha chains having 86 amino acids possess a structure that allows interaction with heme or that heme binding to nascent globin chains promotes formation of the proper tertiary structure of the growing polypeptide chain on polyribosomes ( 19,  20).	transcription
58587	3	335792	5	NULL	NULL	0	NULL	polypeptide chain		growing	forms					tertiary structure					NULL	polyribosomes	0	NULL	NULL	NULL	gw60_jbiolchem_277_16_13415_s_154	11827978	This indicates that nascent alpha chains having 86 amino acids possess a structure that allows interaction with heme or that heme binding to nascent globin chains promotes formation of the proper tertiary structure of the growing polypeptide chain on polyribosomes ( 19,  20).	transcription
58588	4	335792	5	NULL	NULL	0	NULL	statement 2			promotes					statement 3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_16_13415_s_154	11827978	This indicates that nascent alpha chains having 86 amino acids possess a structure that allows interaction with heme or that heme binding to nascent globin chains promotes formation of the proper tertiary structure of the growing polypeptide chain on polyribosomes ( 19,  20).	transcription
79090	1	335792	6	NULL	NULL	0	NULL	Heme	GP		bind					globin chains	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_16_13415_s_154	11827978	This indicates that nascent alpha chains having 86 amino acids possess a structure that allows interaction with heme or that heme binding to nascent globin chains promotes formation of the proper tertiary structure of the growing polypeptide chain on polyribosomes ( 19,  20).	transcription
58594	1	335794	5	NULL	NULL	0	NULL	heme-globin linkage			is present in					hemoglobin			alpha chains		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10130_s_225	8626572	In conclusion, the present data bring out that in  hemoglobin the heme-globin linkage in the alpha  chains is stabilized by  interactions between unlike chains at the alpha beta   interface, whereas heme binding to the beta  chains is stabilized  by interactions at the alpha beta   interface.	transcription
58595	2	335794	5	NULL	NULL	0	NULL	statement 1			is stabilized by					alpha beta interface		interactions between	unlike chains		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10130_s_225	8626572	In conclusion, the present data bring out that in  hemoglobin the heme-globin linkage in the alpha  chains is stabilized by  interactions between unlike chains at the alpha beta   interface, whereas heme binding to the beta  chains is stabilized  by interactions at the alpha beta   interface.	transcription
58596	3	335794	5	NULL	NULL	0	NULL	heme			bind					beta chains					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10130_s_225	8626572	In conclusion, the present data bring out that in  hemoglobin the heme-globin linkage in the alpha  chains is stabilized by  interactions between unlike chains at the alpha beta   interface, whereas heme binding to the beta  chains is stabilized  by interactions at the alpha beta   interface.	transcription
58597	4	335794	5	NULL	NULL	0	NULL	alpha beta interface		interactions at	stabilize					statement 3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10130_s_225	8626572	In conclusion, the present data bring out that in  hemoglobin the heme-globin linkage in the alpha  chains is stabilized by  interactions between unlike chains at the alpha beta   interface, whereas heme binding to the beta  chains is stabilized  by interactions at the alpha beta   interface.	transcription
79091	1	335794	6	NULL	NULL	0	NULL	Heme	GP		bind								beta chain		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_17_10130_s_225	8626572	In conclusion, the present data bring out that in  hemoglobin the heme-globin linkage in the alpha  chains is stabilized by  interactions between unlike chains at the alpha beta   interface, whereas heme binding to the beta  chains is stabilized  by interactions at the alpha beta   interface.	transcription
58598	1	335795	5	NULL	NULL	0	NULL	heme			bind					cytochrome b5			His63		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_6778_s_104	14672943	Based on the heme binding and spectroscopic data for the two axial mutants of cytochrome  b5, we had proposed that His63 plays a primary role for the binding of heme to cytochrome  b5 and acts in a manner analogous to the proximal histidine in globin, while His39 would correspond to the "`distal histidine"`, with ligation of His39 to the heme iron being critical for the electron transfer reaction catalyzed by cytochrome  b5 and not for heme binding ( ).	transcription
58599	2	335795	5	NULL	NULL	0	NULL	cytochrome b5			acts as			His63		globin		proximal	histidine		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_6778_s_104	14672943	Based on the heme binding and spectroscopic data for the two axial mutants of cytochrome  b5, we had proposed that His63 plays a primary role for the binding of heme to cytochrome  b5 and acts in a manner analogous to the proximal histidine in globin, while His39 would correspond to the "`distal histidine"`, with ligation of His39 to the heme iron being critical for the electron transfer reaction catalyzed by cytochrome  b5 and not for heme binding ( ).	transcription
58600	3	335795	5	NULL	NULL	0	NULL	cytochrome b5			corresponds to			His39 		distal histidine					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_6778_s_104	14672943	Based on the heme binding and spectroscopic data for the two axial mutants of cytochrome  b5, we had proposed that His63 plays a primary role for the binding of heme to cytochrome  b5 and acts in a manner analogous to the proximal histidine in globin, while His39 would correspond to the "`distal histidine"`, with ligation of His39 to the heme iron being critical for the electron transfer reaction catalyzed by cytochrome  b5 and not for heme binding ( ).	transcription
58601	4	335795	5	NULL	NULL	0	NULL	electron transfer reaction			is catalyzed by					cytochrome b5					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_6778_s_104	14672943	Based on the heme binding and spectroscopic data for the two axial mutants of cytochrome  b5, we had proposed that His63 plays a primary role for the binding of heme to cytochrome  b5 and acts in a manner analogous to the proximal histidine in globin, while His39 would correspond to the "`distal histidine"`, with ligation of His39 to the heme iron being critical for the electron transfer reaction catalyzed by cytochrome  b5 and not for heme binding ( ).	transcription
58602	5	335795	5	NULL	NULL	0	NULL	cytochrome b5		ligation of	is critical for			His39		statement 4					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_8_6778_s_104	14672943	Based on the heme binding and spectroscopic data for the two axial mutants of cytochrome  b5, we had proposed that His63 plays a primary role for the binding of heme to cytochrome  b5 and acts in a manner analogous to the proximal histidine in globin, while His39 would correspond to the "`distal histidine"`, with ligation of His39 to the heme iron being critical for the electron transfer reaction catalyzed by cytochrome  b5 and not for heme binding ( ).	transcription
58603	1	335800	5	NULL	NULL	0	NULL	bacteria			produce					monocot globin protein					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_27_16746_s_193	9201978	The distinct red color of the recombinant bacteria and the purified protein, as well as its absorbance spectra, is strong evidence that the bacteria can properly produce a monocot globin protein capable of binding heme and constitute definitive evidence that the cloned Hb cDNA does in fact represent a Hb gene.	transcription
58604	2	335800	5	NULL	NULL	0	NULL	monocot globin protein			bind					heme					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_27_16746_s_193	9201978	The distinct red color of the recombinant bacteria and the purified protein, as well as its absorbance spectra, is strong evidence that the bacteria can properly produce a monocot globin protein capable of binding heme and constitute definitive evidence that the cloned Hb cDNA does in fact represent a Hb gene.	transcription
58605	1	335801	5	NULL	NULL	0	NULL	protein kinases			phosphorylates					eIF2alpha			Ser51		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21458_s_21	16717090	Four protein kinases phosphorylate eIF2alpha at Ser51 in response to different stress stimuli: 1) the dsRNA-activated protein kinase PKR is a major component of the interferonmediated antiviral response and is activated by binding to dsRNA produced during viral infection ( ); 2) the general control of nitrogen metabolism kinase GCN2 responds to amino acid depletion ( ); 3) the heme-regulated inhibitor kinase HRI responds to heme deprivation to couple globin synthesis with available heme ( ); and 4) the PKR-related endoplasmic reticulum (ER) kinase PERK responds to the accumulation of unfolded proteins in the ER in a subpathway of the unfolded protein response ( ).	transcription
58606	2	335801	5	NULL	NULL	0	NULL	statement 1			in response to					stress stimuli					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21458_s_21	16717090	Four protein kinases phosphorylate eIF2alpha at Ser51 in response to different stress stimuli: 1) the dsRNA-activated protein kinase PKR is a major component of the interferonmediated antiviral response and is activated by binding to dsRNA produced during viral infection ( ); 2) the general control of nitrogen metabolism kinase GCN2 responds to amino acid depletion ( ); 3) the heme-regulated inhibitor kinase HRI responds to heme deprivation to couple globin synthesis with available heme ( ); and 4) the PKR-related endoplasmic reticulum (ER) kinase PERK responds to the accumulation of unfolded proteins in the ER in a subpathway of the unfolded protein response ( ).	transcription
58607	3	335801	5	NULL	NULL	0	NULL	PKR			is a type of					protein kinase					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21458_s_21	16717090	Four protein kinases phosphorylate eIF2alpha at Ser51 in response to different stress stimuli: 1) the dsRNA-activated protein kinase PKR is a major component of the interferonmediated antiviral response and is activated by binding to dsRNA produced during viral infection ( ); 2) the general control of nitrogen metabolism kinase GCN2 responds to amino acid depletion ( ); 3) the heme-regulated inhibitor kinase HRI responds to heme deprivation to couple globin synthesis with available heme ( ); and 4) the PKR-related endoplasmic reticulum (ER) kinase PERK responds to the accumulation of unfolded proteins in the ER in a subpathway of the unfolded protein response ( ).	transcription
58608	4	335801	5	NULL	NULL	0	NULL	PKR			is activated by					dsRNA					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21458_s_21	16717090	Four protein kinases phosphorylate eIF2alpha at Ser51 in response to different stress stimuli: 1) the dsRNA-activated protein kinase PKR is a major component of the interferonmediated antiviral response and is activated by binding to dsRNA produced during viral infection ( ); 2) the general control of nitrogen metabolism kinase GCN2 responds to amino acid depletion ( ); 3) the heme-regulated inhibitor kinase HRI responds to heme deprivation to couple globin synthesis with available heme ( ); and 4) the PKR-related endoplasmic reticulum (ER) kinase PERK responds to the accumulation of unfolded proteins in the ER in a subpathway of the unfolded protein response ( ).	transcription
58609	5	335801	5	NULL	NULL	0	NULL	antiviral response			is mediated by					interferon					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21458_s_21	16717090	Four protein kinases phosphorylate eIF2alpha at Ser51 in response to different stress stimuli: 1) the dsRNA-activated protein kinase PKR is a major component of the interferonmediated antiviral response and is activated by binding to dsRNA produced during viral infection ( ); 2) the general control of nitrogen metabolism kinase GCN2 responds to amino acid depletion ( ); 3) the heme-regulated inhibitor kinase HRI responds to heme deprivation to couple globin synthesis with available heme ( ); and 4) the PKR-related endoplasmic reticulum (ER) kinase PERK responds to the accumulation of unfolded proteins in the ER in a subpathway of the unfolded protein response ( ).	transcription
58610	6	335801	5	NULL	NULL	0	NULL	PKR			is a component of		major			statement 5					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21458_s_21	16717090	Four protein kinases phosphorylate eIF2alpha at Ser51 in response to different stress stimuli: 1) the dsRNA-activated protein kinase PKR is a major component of the interferonmediated antiviral response and is activated by binding to dsRNA produced during viral infection ( ); 2) the general control of nitrogen metabolism kinase GCN2 responds to amino acid depletion ( ); 3) the heme-regulated inhibitor kinase HRI responds to heme deprivation to couple globin synthesis with available heme ( ); and 4) the PKR-related endoplasmic reticulum (ER) kinase PERK responds to the accumulation of unfolded proteins in the ER in a subpathway of the unfolded protein response ( ).	transcription
58611	7	335801	5	NULL	NULL	0	NULL	dsRNA			is produced during					virus		infection of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21458_s_21	16717090	Four protein kinases phosphorylate eIF2alpha at Ser51 in response to different stress stimuli: 1) the dsRNA-activated protein kinase PKR is a major component of the interferonmediated antiviral response and is activated by binding to dsRNA produced during viral infection ( ); 2) the general control of nitrogen metabolism kinase GCN2 responds to amino acid depletion ( ); 3) the heme-regulated inhibitor kinase HRI responds to heme deprivation to couple globin synthesis with available heme ( ); and 4) the PKR-related endoplasmic reticulum (ER) kinase PERK responds to the accumulation of unfolded proteins in the ER in a subpathway of the unfolded protein response ( ).	transcription
58612	8	335801	5	NULL	NULL	0	NULL	PKR			bind					statement 7					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21458_s_21	16717090	Four protein kinases phosphorylate eIF2alpha at Ser51 in response to different stress stimuli: 1) the dsRNA-activated protein kinase PKR is a major component of the interferonmediated antiviral response and is activated by binding to dsRNA produced during viral infection ( ); 2) the general control of nitrogen metabolism kinase GCN2 responds to amino acid depletion ( ); 3) the heme-regulated inhibitor kinase HRI responds to heme deprivation to couple globin synthesis with available heme ( ); and 4) the PKR-related endoplasmic reticulum (ER) kinase PERK responds to the accumulation of unfolded proteins in the ER in a subpathway of the unfolded protein response ( ).	transcription
58613	9	335801	5	NULL	NULL	0	NULL	statement 8			activates					PKR					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21458_s_21	16717090	Four protein kinases phosphorylate eIF2alpha at Ser51 in response to different stress stimuli: 1) the dsRNA-activated protein kinase PKR is a major component of the interferonmediated antiviral response and is activated by binding to dsRNA produced during viral infection ( ); 2) the general control of nitrogen metabolism kinase GCN2 responds to amino acid depletion ( ); 3) the heme-regulated inhibitor kinase HRI responds to heme deprivation to couple globin synthesis with available heme ( ); and 4) the PKR-related endoplasmic reticulum (ER) kinase PERK responds to the accumulation of unfolded proteins in the ER in a subpathway of the unfolded protein response ( ).	transcription
58614	10	335801	5	NULL	NULL	0	NULL	GCN2			is a type of					nitrogen metabolism					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21458_s_21	16717090	Four protein kinases phosphorylate eIF2alpha at Ser51 in response to different stress stimuli: 1) the dsRNA-activated protein kinase PKR is a major component of the interferonmediated antiviral response and is activated by binding to dsRNA produced during viral infection ( ); 2) the general control of nitrogen metabolism kinase GCN2 responds to amino acid depletion ( ); 3) the heme-regulated inhibitor kinase HRI responds to heme deprivation to couple globin synthesis with available heme ( ); and 4) the PKR-related endoplasmic reticulum (ER) kinase PERK responds to the accumulation of unfolded proteins in the ER in a subpathway of the unfolded protein response ( ).	transcription
58615	11	335801	5	NULL	NULL	0	NULL	GCN2		control of	respond to					amino acid		depletion of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21458_s_21	16717090	Four protein kinases phosphorylate eIF2alpha at Ser51 in response to different stress stimuli: 1) the dsRNA-activated protein kinase PKR is a major component of the interferonmediated antiviral response and is activated by binding to dsRNA produced during viral infection ( ); 2) the general control of nitrogen metabolism kinase GCN2 responds to amino acid depletion ( ); 3) the heme-regulated inhibitor kinase HRI responds to heme deprivation to couple globin synthesis with available heme ( ); and 4) the PKR-related endoplasmic reticulum (ER) kinase PERK responds to the accumulation of unfolded proteins in the ER in a subpathway of the unfolded protein response ( ).	transcription
58616	12	335801	5	NULL	NULL	0	NULL	HRI 			is					heme-regulated inhibitor kinase					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_21458_s_21	16717090	Four protein kinases phosphorylate eIF2alpha at Ser51 in response to different stress stimuli: 1) the dsRNA-activated protein kinase PKR is a major component of the interferonmediated antiviral response and is activated by binding to dsRNA produced during viral infection ( ); 2) the general control of nitrogen metabolism kinase GCN2 responds to amino acid depletion ( ); 3) the heme-regulated inhibitor kinase HRI responds to heme deprivation to couple globin synthesis with available heme ( ); and 4) the PKR-related endoplasmic reticulum (ER) kinase PERK responds to the accumulation of unfolded proteins in the ER in a subpathway of the unfolded protein response ( ).	transcription
58617	13	335801	5	NULL	NULL	0	NULL	PERK			is					PKR-related endoplasmic reticulum (ER) kinase					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_30_21458_s_21	16717090	Four protein kinases phosphorylate eIF2alpha at Ser51 in response to different stress stimuli: 1) the dsRNA-activated protein kinase PKR is a major component of the interferonmediated antiviral response and is activated by binding to dsRNA produced during viral infection ( ); 2) the general control of nitrogen metabolism kinase GCN2 responds to amino acid depletion ( ); 3) the heme-regulated inhibitor kinase HRI responds to heme deprivation to couple globin synthesis with available heme ( ); and 4) the PKR-related endoplasmic reticulum (ER) kinase PERK responds to the accumulation of unfolded proteins in the ER in a subpathway of the unfolded protein response ( ).	transcription
58618	14	335801	5	NULL	NULL	0	NULL	HRI			respond to					heme		deprivation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21458_s_21	16717090	Four protein kinases phosphorylate eIF2alpha at Ser51 in response to different stress stimuli: 1) the dsRNA-activated protein kinase PKR is a major component of the interferonmediated antiviral response and is activated by binding to dsRNA produced during viral infection ( ); 2) the general control of nitrogen metabolism kinase GCN2 responds to amino acid depletion ( ); 3) the heme-regulated inhibitor kinase HRI responds to heme deprivation to couple globin synthesis with available heme ( ); and 4) the PKR-related endoplasmic reticulum (ER) kinase PERK responds to the accumulation of unfolded proteins in the ER in a subpathway of the unfolded protein response ( ).	transcription
58619	15	335801	5	NULL	NULL	0	NULL	HRI			is coupled to					globin synthesis					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21458_s_21	16717090	Four protein kinases phosphorylate eIF2alpha at Ser51 in response to different stress stimuli: 1) the dsRNA-activated protein kinase PKR is a major component of the interferonmediated antiviral response and is activated by binding to dsRNA produced during viral infection ( ); 2) the general control of nitrogen metabolism kinase GCN2 responds to amino acid depletion ( ); 3) the heme-regulated inhibitor kinase HRI responds to heme deprivation to couple globin synthesis with available heme ( ); and 4) the PKR-related endoplasmic reticulum (ER) kinase PERK responds to the accumulation of unfolded proteins in the ER in a subpathway of the unfolded protein response ( ).	transcription
58620	16	335801	5	NULL	NULL	0	NULL	statement 15			occurs with					heme		available			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21458_s_21	16717090	Four protein kinases phosphorylate eIF2alpha at Ser51 in response to different stress stimuli: 1) the dsRNA-activated protein kinase PKR is a major component of the interferonmediated antiviral response and is activated by binding to dsRNA produced during viral infection ( ); 2) the general control of nitrogen metabolism kinase GCN2 responds to amino acid depletion ( ); 3) the heme-regulated inhibitor kinase HRI responds to heme deprivation to couple globin synthesis with available heme ( ); and 4) the PKR-related endoplasmic reticulum (ER) kinase PERK responds to the accumulation of unfolded proteins in the ER in a subpathway of the unfolded protein response ( ).	transcription
58621	17	335801	5	NULL	NULL	0	NULL	statement 16			occurs simultaneously with					statement 14					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21458_s_21	16717090	Four protein kinases phosphorylate eIF2alpha at Ser51 in response to different stress stimuli: 1) the dsRNA-activated protein kinase PKR is a major component of the interferonmediated antiviral response and is activated by binding to dsRNA produced during viral infection ( ); 2) the general control of nitrogen metabolism kinase GCN2 responds to amino acid depletion ( ); 3) the heme-regulated inhibitor kinase HRI responds to heme deprivation to couple globin synthesis with available heme ( ); and 4) the PKR-related endoplasmic reticulum (ER) kinase PERK responds to the accumulation of unfolded proteins in the ER in a subpathway of the unfolded protein response ( ).	transcription
58622	18	335801	5	NULL	NULL	0	NULL	PERK			respond to					unfolded proteins		accumulation of			NULL	ER	0	NULL	NULL	NULL	gw70_jbiolchem_281_30_21458_s_21	16717090	Four protein kinases phosphorylate eIF2alpha at Ser51 in response to different stress stimuli: 1) the dsRNA-activated protein kinase PKR is a major component of the interferonmediated antiviral response and is activated by binding to dsRNA produced during viral infection ( ); 2) the general control of nitrogen metabolism kinase GCN2 responds to amino acid depletion ( ); 3) the heme-regulated inhibitor kinase HRI responds to heme deprivation to couple globin synthesis with available heme ( ); and 4) the PKR-related endoplasmic reticulum (ER) kinase PERK responds to the accumulation of unfolded proteins in the ER in a subpathway of the unfolded protein response ( ).	transcription
58623	1	335802	5	NULL	NULL	0	NULL	globin		synthesis of	modulated by					heme-regulated translational inhibitor					NULL		0	NULL	NULL	NULL	abs-batch0650-0679_biol-res_39_1_16629165_s_3	16629165	For example, three enzymes involved in erythrocyte  development are regulated by three different control mechanisms: globin  synthesis is modulated by heme-regulated translational inhibitor, erythroid  5-aminolevulinate synthase translation is inhibited by binding of the  iron regulatory protein to the iron response element in the 5''-untranslated  region (UTR); and 15-lipoxygenase is regulated by specific proteins binding  to the 3''-UTR.	transcription
58624	2	335802	5	NULL	NULL	0	NULL	iron regulatory protein			bind									iron response element in 5'' -UTR	NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_biol-res_39_1_16629165_s_3	16629165	For example, three enzymes involved in erythrocyte  development are regulated by three different control mechanisms: globin  synthesis is modulated by heme-regulated translational inhibitor, erythroid  5-aminolevulinate synthase translation is inhibited by binding of the  iron regulatory protein to the iron response element in the 5''-untranslated  region (UTR); and 15-lipoxygenase is regulated by specific proteins binding  to the 3''-UTR.	transcription
58625	3	335802	5	NULL	NULL	0	NULL	statement 2			inhibits					5-aminolevulinate synthase		erythroid			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_biol-res_39_1_16629165_s_3	16629165	For example, three enzymes involved in erythrocyte  development are regulated by three different control mechanisms: globin  synthesis is modulated by heme-regulated translational inhibitor, erythroid  5-aminolevulinate synthase translation is inhibited by binding of the  iron regulatory protein to the iron response element in the 5''-untranslated  region (UTR); and 15-lipoxygenase is regulated by specific proteins binding  to the 3''-UTR.	transcription
58626	4	335802	5	NULL	NULL	0	NULL	proteins 		specific 	bind									3''-UTR	NULL		0	NULL	NULL	NULL	abs-batch0650-0679_biol-res_39_1_16629165_s_3	16629165	For example, three enzymes involved in erythrocyte  development are regulated by three different control mechanisms: globin  synthesis is modulated by heme-regulated translational inhibitor, erythroid  5-aminolevulinate synthase translation is inhibited by binding of the  iron regulatory protein to the iron response element in the 5''-untranslated  region (UTR); and 15-lipoxygenase is regulated by specific proteins binding  to the 3''-UTR.	transcription
58627	5	335802	5	NULL	NULL	0	NULL	statement 4			regulates					15-lipoxygenase					NULL		0	NULL	NULL	NULL	abs-batch0650-0679_biol-res_39_1_16629165_s_3	16629165	For example, three enzymes involved in erythrocyte  development are regulated by three different control mechanisms: globin  synthesis is modulated by heme-regulated translational inhibitor, erythroid  5-aminolevulinate synthase translation is inhibited by binding of the  iron regulatory protein to the iron response element in the 5''-untranslated  region (UTR); and 15-lipoxygenase is regulated by specific proteins binding  to the 3''-UTR.	transcription
79103	1	335802	6	NULL	NULL	0	NULL	globin	GP	synthesis of	is modulated by					heme-regulated translational inhibitor					NULL		0	NULL	NULL	NULL	abs-batch0650-0679_biol-res_39_1_16629165_s_3	16629165	For example, three enzymes involved in erythrocyte  development are regulated by three different control mechanisms: globin  synthesis is modulated by heme-regulated translational inhibitor, erythroid  5-aminolevulinate synthase translation is inhibited by binding of the  iron regulatory protein to the iron response element in the 5''-untranslated  region (UTR); and 15-lipoxygenase is regulated by specific proteins binding  to the 3''-UTR.	transcription
79104	3	335802	6	NULL	NULL	0	NULL	erythroid 5-aminolevulinate synthase	GP	translation of 	is inhibited by					statement 2	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_biol-res_39_1_16629165_s_3	16629165	For example, three enzymes involved in erythrocyte  development are regulated by three different control mechanisms: globin  synthesis is modulated by heme-regulated translational inhibitor, erythroid  5-aminolevulinate synthase translation is inhibited by binding of the  iron regulatory protein to the iron response element in the 5''-untranslated  region (UTR); and 15-lipoxygenase is regulated by specific proteins binding  to the 3''-UTR.	transcription
79105	2	335802	6	NULL	NULL	0	NULL	iron regulatory protein	GP		bind									iron response element in the 5''-untranslated region (UTR)	NULL		0	NULL	NULL	NULL	abs-batch0650-0679_biol-res_39_1_16629165_s_3	16629165	For example, three enzymes involved in erythrocyte  development are regulated by three different control mechanisms: globin  synthesis is modulated by heme-regulated translational inhibitor, erythroid  5-aminolevulinate synthase translation is inhibited by binding of the  iron regulatory protein to the iron response element in the 5''-untranslated  region (UTR); and 15-lipoxygenase is regulated by specific proteins binding  to the 3''-UTR.	transcription
58628	1	335803	5	NULL	NULL	0	NULL	taurine			interacts with					hypochlorite anion					NULL		0	NULL	NULL	NULL	abs-batch0760-0779_biull-eksp-biol-med_114_11_1337841_s_1	1337841	[The interaction of taurine and beta-alanyl-L-histidine (carnosine) with hypochlorite anion (ClO-)].	transcription
58629	2	335803	5	NULL	NULL	0	NULL	beta-alanyl-L-histidine			interacts with					hypochlorite anion					NULL		0	NULL	NULL	NULL	abs-batch0760-0779_biull-eksp-biol-med_114_11_1337841_s_1	1337841	[The interaction of taurine and beta-alanyl-L-histidine (carnosine) with hypochlorite anion (ClO-)].	transcription
58630	3	335803	5	NULL	NULL	0	NULL	beta-alanyl-L-histidine			is					carnosine					NULL		0	NULL	NULL	NULL	abs-batch0760-0779_biull-eksp-biol-med_114_11_1337841_s_1	1337841	[The interaction of taurine and beta-alanyl-L-histidine (carnosine) with hypochlorite anion (ClO-)].	transcription
58631	4	335803	5	NULL	NULL	0	NULL	hypochlorite anion			is					ClO-					NULL		0	NULL	NULL	NULL	abs-batch0760-0779_biull-eksp-biol-med_114_11_1337841_s_1	1337841	[The interaction of taurine and beta-alanyl-L-histidine (carnosine) with hypochlorite anion (ClO-)].	transcription
79157	1	335803	6	NULL	NULL	0	NULL	taurine	AminoAcid		bind					beta-alanyl-L-histidine	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0760-0779_biull-eksp-biol-med_114_11_1337841_s_1	1337841	[The interaction of taurine and beta-alanyl-L-histidine (carnosine) with hypochlorite anion (ClO-)].	transcription
79158	2	335803	6	NULL	NULL	0	NULL	beta-alanyl-L-histidine	Chemical		is					carnosine	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0760-0779_biull-eksp-biol-med_114_11_1337841_s_1	1337841	[The interaction of taurine and beta-alanyl-L-histidine (carnosine) with hypochlorite anion (ClO-)].	transcription
58632	1	335804	5	NULL	NULL	0	NULL	CE		activity of	release					beta-alanine					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_8_3540_s_161	10427046	The activity of CE mainly released beta-alanine, histidine, alanine, and anserine, while the levels of glycine, glutamine, and carnosine decreased.	transcription
58633	2	335804	5	NULL	NULL	0	NULL	CE		activity of	release					histidine					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_8_3540_s_161	10427046	The activity of CE mainly released beta-alanine, histidine, alanine, and anserine, while the levels of glycine, glutamine, and carnosine decreased.	transcription
58634	3	335804	5	NULL	NULL	0	NULL	CE		activity of	release					alanine					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_8_3540_s_161	10427046	The activity of CE mainly released beta-alanine, histidine, alanine, and anserine, while the levels of glycine, glutamine, and carnosine decreased.	transcription
58635	4	335804	5	NULL	NULL	0	NULL	CE		activity of	release					anserine					NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_8_3540_s_161	10427046	The activity of CE mainly released beta-alanine, histidine, alanine, and anserine, while the levels of glycine, glutamine, and carnosine decreased.	transcription
58636	5	335804	5	NULL	NULL	0	NULL	CE		activity of	decreases					glycine		level of			NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_65_8_3540_s_161	10427046	The activity of CE mainly released beta-alanine, histidine, alanine, and anserine, while the levels of glycine, glutamine, and carnosine decreased.	transcription
58637	6	335804	5	NULL	NULL	0	NULL	CE		activity of	decreases					glutamine		level of			NULL		NULL	NULL	NULL	NULL	gw60_applenvironmicrob_65_8_3540_s_161	10427046	The activity of CE mainly released beta-alanine, histidine, alanine, and anserine, while the levels of glycine, glutamine, and carnosine decreased.	transcription
58638	7	335804	5	NULL	NULL	0	NULL	CE		activity of	decreases					carnosine 		level of			NULL		0	NULL	NULL	NULL	gw60_applenvironmicrob_65_8_3540_s_161	10427046	The activity of CE mainly released beta-alanine, histidine, alanine, and anserine, while the levels of glycine, glutamine, and carnosine decreased.	transcription
58639	1	335805	5	NULL	NULL	0	NULL	Carnosine			is					beta-alanyl-L-histidine					NULL		0	NULL	NULL	NULL	abs-batch0760-0779_biull-eksp-biol-med_107_2_2923966_s_2	2923966	Carnosine (beta-alanyl-L-histidine) injected to intact albino rats (20  mg/kg body weight) induces depletion of lipid peroxidation (LPO) products  in brain and blood serum, an increase of superoxide scavenging activity  in brain and serum, decrease of cholesterol: phospholipid ratio and increase  of easy oxidizable phospholipid portion in brain lipid extracts.	transcription
58640	2	335805	5	NULL	NULL	0	NULL	Carnosine			is injected to					albino rats		intact			NULL		0	NULL	NULL	NULL	abs-batch0760-0779_biull-eksp-biol-med_107_2_2923966_s_2	2923966	Carnosine (beta-alanyl-L-histidine) injected to intact albino rats (20  mg/kg body weight) induces depletion of lipid peroxidation (LPO) products  in brain and blood serum, an increase of superoxide scavenging activity  in brain and serum, decrease of cholesterol: phospholipid ratio and increase  of easy oxidizable phospholipid portion in brain lipid extracts.	transcription
58641	3	335805	5	NULL	NULL	0	NULL	statement 2			induce					LPO products		depletion of			NULL	brain, blood serum	NULL	NULL	NULL	NULL	abs-batch0760-0779_biull-eksp-biol-med_107_2_2923966_s_2	2923966	Carnosine (beta-alanyl-L-histidine) injected to intact albino rats (20  mg/kg body weight) induces depletion of lipid peroxidation (LPO) products  in brain and blood serum, an increase of superoxide scavenging activity  in brain and serum, decrease of cholesterol: phospholipid ratio and increase  of easy oxidizable phospholipid portion in brain lipid extracts.	transcription
58642	4	335805	5	NULL	NULL	0	NULL	LPO products			is					lipid peroxidation products					NULL		0	NULL	NULL	NULL	abs-batch0760-0779_biull-eksp-biol-med_107_2_2923966_s_2	2923966	Carnosine (beta-alanyl-L-histidine) injected to intact albino rats (20  mg/kg body weight) induces depletion of lipid peroxidation (LPO) products  in brain and blood serum, an increase of superoxide scavenging activity  in brain and serum, decrease of cholesterol: phospholipid ratio and increase  of easy oxidizable phospholipid portion in brain lipid extracts.	transcription
58643	5	335805	5	NULL	NULL	0	NULL	statement 2			increases					superoxide		scavenging activity of			NULL	brain, blood serum	0	NULL	NULL	NULL	abs-batch0760-0779_biull-eksp-biol-med_107_2_2923966_s_2	2923966	Carnosine (beta-alanyl-L-histidine) injected to intact albino rats (20  mg/kg body weight) induces depletion of lipid peroxidation (LPO) products  in brain and blood serum, an increase of superoxide scavenging activity  in brain and serum, decrease of cholesterol: phospholipid ratio and increase  of easy oxidizable phospholipid portion in brain lipid extracts.	transcription
58644	6	335805	5	NULL	NULL	0	NULL	statement 2			decreases					cholesterol: phospholipid ratio					NULL		NULL	NULL	NULL	NULL	abs-batch0760-0779_biull-eksp-biol-med_107_2_2923966_s_2	2923966	Carnosine (beta-alanyl-L-histidine) injected to intact albino rats (20  mg/kg body weight) induces depletion of lipid peroxidation (LPO) products  in brain and blood serum, an increase of superoxide scavenging activity  in brain and serum, decrease of cholesterol: phospholipid ratio and increase  of easy oxidizable phospholipid portion in brain lipid extracts.	transcription
58645	7	335805	5	NULL	NULL	0	NULL	statement 2			increases					phospholipid portion		easy oxidizable			NULL	brain lipid extracts	0	NULL	NULL	NULL	abs-batch0760-0779_biull-eksp-biol-med_107_2_2923966_s_2	2923966	Carnosine (beta-alanyl-L-histidine) injected to intact albino rats (20  mg/kg body weight) induces depletion of lipid peroxidation (LPO) products  in brain and blood serum, an increase of superoxide scavenging activity  in brain and serum, decrease of cholesterol: phospholipid ratio and increase  of easy oxidizable phospholipid portion in brain lipid extracts.	transcription
79159	1	335805	6	NULL	NULL	0	NULL	beta-alanyl-L-histidine	AminoAcid		induces					LPO	Process	depletion of 			NULL		0	NULL	NULL	NULL	abs-batch0760-0779_biull-eksp-biol-med_107_2_2923966_s_2	2923966	Carnosine (beta-alanyl-L-histidine) injected to intact albino rats (20  mg/kg body weight) induces depletion of lipid peroxidation (LPO) products  in brain and blood serum, an increase of superoxide scavenging activity  in brain and serum, decrease of cholesterol: phospholipid ratio and increase  of easy oxidizable phospholipid portion in brain lipid extracts.	transcription
79160	2	335805	6	NULL	NULL	0	NULL	beta-alanyl-L-histidine	AminoAcid		is					carnosine	AminoAcid				NULL		0	NULL	NULL	NULL	abs-batch0760-0779_biull-eksp-biol-med_107_2_2923966_s_2	2923966	Carnosine (beta-alanyl-L-histidine) injected to intact albino rats (20  mg/kg body weight) induces depletion of lipid peroxidation (LPO) products  in brain and blood serum, an increase of superoxide scavenging activity  in brain and serum, decrease of cholesterol: phospholipid ratio and increase  of easy oxidizable phospholipid portion in brain lipid extracts.	transcription
79161	3	335805	6	NULL	NULL	NULL	NULL	beta-alanyl-L-histidine	AminoAcid		increases					superoxide scavenging activity	Process				NULL	brain	NULL	NULL	NULL	NULL	abs-batch0760-0779_biull-eksp-biol-med_107_2_2923966_s_2	2923966	Carnosine (beta-alanyl-L-histidine) injected to intact albino rats (20  mg/kg body weight) induces depletion of lipid peroxidation (LPO) products  in brain and blood serum, an increase of superoxide scavenging activity  in brain and serum, decrease of cholesterol: phospholipid ratio and increase  of easy oxidizable phospholipid portion in brain lipid extracts.	transcription
79162	4	335805	6	NULL	NULL	0	NULL	beta-alanyl-L-histidine	AminoAcid		increases					superoxide scavenging activity	Process				NULL	serum	0	NULL	NULL	NULL	abs-batch0760-0779_biull-eksp-biol-med_107_2_2923966_s_2	2923966	Carnosine (beta-alanyl-L-histidine) injected to intact albino rats (20  mg/kg body weight) induces depletion of lipid peroxidation (LPO) products  in brain and blood serum, an increase of superoxide scavenging activity  in brain and serum, decrease of cholesterol: phospholipid ratio and increase  of easy oxidizable phospholipid portion in brain lipid extracts.	transcription
79163	5	335805	6	NULL	NULL	0	NULL	beta-alanyl-L-histidine	AminoAcid		induces					cholesterol	Chemical	decrease of 			NULL		0	NULL	NULL	NULL	abs-batch0760-0779_biull-eksp-biol-med_107_2_2923966_s_2	2923966	Carnosine (beta-alanyl-L-histidine) injected to intact albino rats (20  mg/kg body weight) induces depletion of lipid peroxidation (LPO) products  in brain and blood serum, an increase of superoxide scavenging activity  in brain and serum, decrease of cholesterol: phospholipid ratio and increase  of easy oxidizable phospholipid portion in brain lipid extracts.	transcription
58646	1	335806	5	NULL	NULL	0	NULL	fimbriae		purified	bind					glucosylceramide					NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58647	2	335806	5	NULL	NULL	0	NULL	glucosylceramide			is					GlcCer					NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58648	3	335806	5	NULL	NULL	0	NULL	fimbriae		purified	bind					galactosylceramide 2					NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58649	4	335806	5	NULL	NULL	0	NULL	galactosylceramide 2			is a type of					nonhydroxylated fatty acids					NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58650	5	335806	5	NULL	NULL	0	NULL	fimbriae		purified	bind					lactosylceramide					NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58651	6	335806	5	NULL	NULL	0	NULL	lactosylceramide			is					LacCer					NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58652	7	335806	5	NULL	NULL	0	NULL	fimbriae		purified	bind					paragloboside					NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58653	8	335806	5	NULL	NULL	0	NULL	paragloboside			is					nLc4Cer					NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58654	9	335806	5	NULL	NULL	0	NULL	fimbriae		purified	bind					lactotriaosylceramide					NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58655	10	335806	5	NULL	NULL	0	NULL	lactotriaosylceramide			is					Lc3Cer					NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58656	11	335806	5	NULL	NULL	0	NULL	fimbriae		purified	bind					asialo-GM1					NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58657	12	335806	5	NULL	NULL	0	NULL	asialo-GM1			is					GgO4Cer					NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58658	13	335806	5	NULL	NULL	0	NULL	fimbriae		purified	bind					asialo-GM2					NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58659	14	335806	5	NULL	NULL	0	NULL	asialo-GM2			is					GgO3Cer					NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58660	15	335806	5	NULL	NULL	0	NULL	fimbriae		purified	bind					globotriaosylceramide					NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58661	16	335806	5	NULL	NULL	0	NULL	globotriaosylceramide			is					Gb3Cer					NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58662	17	335806	5	NULL	NULL	0	NULL	fimbriae		purified	does not bind					sulfatide 					NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58663	18	335806	5	NULL	NULL	0	NULL	sulfatide 			is					SFT					NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58664	19	335806	5	NULL	NULL	0	NULL	fimbriae		purified	does not bind					globotetraosylceramide					NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58665	20	335806	5	NULL	NULL	0	NULL	globotetraosylceramide 			is					Gb4Cer					NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58666	21	335806	5	NULL	NULL	0	NULL	fimbriae		purified	does not bind					Forssman antigen					NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58667	22	335806	5	NULL	NULL	0	NULL	fimbriae		purified	does not bind					GM1 					NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58668	23	335806	5	NULL	NULL	0	NULL	fimbriae		purified	does not bind					GM2					NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58669	24	335806	5	NULL	NULL	0	NULL	fimbriae		purified	does not bind					GM3					NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58670	25	335806	5	NULL	NULL	0	NULL	fimbriae		purified	does not bind					GD2					NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58671	26	335806	5	NULL	NULL	0	NULL	fimbriae		purified	does not bind					GD3 					NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58672	27	335806	5	NULL	NULL	0	NULL	fimbriae		purified	does not bind					DSPG					NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58673	28	335806	5	NULL	NULL	0	NULL	fimbriae		purified	does not bind					DSnHC					NULL		NULL	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58674	29	335806	5	NULL	NULL	0	NULL	fimbriae		purified	does not bind					DSnOC 					NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58675	30	335806	5	NULL	NULL	0	NULL	fimbriae		purified	does not bind					ceramide 					NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58676	31	335806	5	NULL	NULL	0	NULL	ceramide 			is					Cer					NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
79164	1	335806	6	NULL	NULL	0	NULL	fimbriae	CellComponent	purified	bind					GlcCer	Chemical				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
79165	2	335806	6	NULL	NULL	0	NULL	fimbriae	CellComponent	purified	bind					nonhydroxylated fatty acids	Chemical				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
79166	3	335806	6	NULL	NULL	0	NULL	fimbriae	CellComponent	purified	bind					LacCer	Chemical				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
79167	4	335806	6	NULL	NULL	0	NULL	fimbriae	CellComponent	purified	bind					nLc4Cer	Chemical				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
79168	5	335806	6	NULL	NULL	0	NULL	fimbriae	CellComponent	purified	bind					Lc3Cer	Chemical				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
79169	6	335806	6	NULL	NULL	0	NULL	fimbriae	CellComponent	purified	bind					GgO4Cer	Chemical				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
79170	7	335806	6	NULL	NULL	0	NULL	fimbriae	CellComponent	purified	bind					GgO3Cer	Chemical				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
79171	8	335806	6	NULL	NULL	0	NULL	fimbriae	CellComponent	purified	bind					Gb3Cer	Chemical				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
79172	9	335806	6	NULL	NULL	0	NULL	GlcCer	Chemical		is					glucosylceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
79173	10	335806	6	NULL	NULL	0	NULL	nonhydroxylated fatty acids	Chemical		is					galactosylceramide 2	Chemical				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
79174	11	335806	6	NULL	NULL	0	NULL	LacCer	Chemical		is					lactosylceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
79175	12	335806	6	NULL	NULL	0	NULL	nLc4Cer	Chemical		is					paragloboside	Chemical				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
79176	13	335806	6	NULL	NULL	0	NULL	Lc3Cer	Chemical		is					lactotriaosylceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
79177	14	335806	6	NULL	NULL	0	NULL	GgO4Cer	Chemical		is					asialo-GM1	Chemical				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
79178	15	335806	6	NULL	NULL	0	NULL	GgO3Cer	Chemical		is					asialo-GM2	Chemical				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
79179	16	335806	6	NULL	NULL	0	NULL	Gb3Cer	Chemical		is					globotriaosylceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
79180	17	335806	6	NULL	NULL	0	NULL	sulfatide	Chemical		is					SFT	Chemical				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
79181	18	335806	6	NULL	NULL	0	NULL	Gb4Cer	Chemical		is					globotetraosylceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
79182	19	335806	6	NULL	NULL	0	NULL	fimbriae	CellComponent	purified	does not bind					Forssman antigen	GP				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
79183	20	335806	6	NULL	NULL	0	NULL	fimbriae	CellComponent	purified	does not bind					SFT	Chemical				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
79184	21	335806	6	NULL	NULL	0	NULL	fimbriae	CellComponent	purified	does not bind					Gb4Cer	GP				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
79185	22	335806	6	NULL	NULL	0	NULL	fimbriae	CellComponent	purified	does not bind					GM1	GP				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
79186	23	335806	6	NULL	NULL	0	NULL	fimbriae	CellComponent	purified	does not bind					GM2	GP				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
79187	24	335806	6	NULL	NULL	0	NULL	fimbriae	CellComponent	purified	does not bind					GM3	Chemical				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
79188	25	335806	6	NULL	NULL	0	NULL	fimbriae	CellComponent	purified	does not bind					GD2	Chemical				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
79189	26	335806	6	NULL	NULL	0	NULL	fimbriae	CellComponent	purified	does not bind					GD2	Chemical				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
79190	27	335806	6	NULL	NULL	0	NULL	fimbriae	CellComponent	purified	does not bind					DSPG	Chemical				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
79191	28	335806	6	NULL	NULL	0	NULL	fimbriae	CellComponent	purified	does not bind					DSnHC	Chemical				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
79192	29	335806	6	NULL	NULL	0	NULL	fimbriae	CellComponent	purified	does not bind					DSnOC	Chemical				NULL		0	NULL	NULL	NULL	gw60_infectimmun_68_6_3541_s_109	10816509	Purified fimbriae bound to glucosylceramide (GlcCer), galactosylceramide 2 (nonhydroxylated fatty acids), lactosylceramide (LacCer), paragloboside (nLc4Cer), lactotriaosylceramide (Lc3Cer), asialo-GM1 (GgO4Cer), asialo-GM2 (GgO3Cer), and globotriaosylceramide (Gb3Cer) (Table  1) but did not bind to sulfatide (SFT), globotetraosylceramide (Gb4Cer), the Forssman antigen (Table  1), GM1 (Fig.  1), GM2, GM3, GD2, GD3 (Table  1), DSPG, DSnHC, DSnOC (see Fig.  3), or ceramide (Cer) (Table  1).	transcription
58677	1	335807	5	NULL	NULL	0	NULL	p73			induce					Bax		up-regulation of			NULL	Saos-2 cells	0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_96	14634023	p73 induces Bax up-regulation in Saos-2 cells.	transcription
79193	1	335807	6	NULL	NULL	0	NULL	p73	GP		induces					Bax	GP	upregulation of			NULL	Saos-2 cells	0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_96	14634023	p73 induces Bax up-regulation in Saos-2 cells.	transcription
58678	1	335808	5	NULL	NULL	0	NULL	p73 isoforms			activates		transcriptionaly			Bax					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_97	14634023	A, Bax transcriptional activation by different p73 isoforms.	transcription
79194	1	335808	6	NULL	NULL	0	NULL	p73	GP		activates					Bax	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_97	14634023	A, Bax transcriptional activation by different p73 isoforms.	transcription
58679	1	335809	5	NULL	NULL	0	NULL	Bax			is translocated from					cytosol					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_122	14634023	p73 induces Bax translocation from cytosol to mitochondria.	transcription
58680	2	335809	5	NULL	NULL	0	NULL	Bax			is translocated to					mitochondria					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_122	14634023	p73 induces Bax translocation from cytosol to mitochondria.	transcription
58681	3	335809	5	NULL	NULL	0	NULL	statement 1			occurs simultaneously with					statement 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_122	14634023	p73 induces Bax translocation from cytosol to mitochondria.	transcription
58682	4	335809	5	NULL	NULL	0	NULL	p73			induce					statement 3					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_122	14634023	p73 induces Bax translocation from cytosol to mitochondria.	transcription
79195	1	335809	6	NULL	NULL	0	NULL	Bax	GP		is translocated from					cytosol	CellComponent				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_122	14634023	p73 induces Bax translocation from cytosol to mitochondria.	transcription
79196	2	335809	6	NULL	NULL	0	NULL	Bax	GP		is translocated to					mitochondria	CellComponent				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_122	14634023	p73 induces Bax translocation from cytosol to mitochondria.	transcription
79197	3	335809	6	NULL	NULL	0	NULL	statement 1	Process		occurs simultaneously with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_122	14634023	p73 induces Bax translocation from cytosol to mitochondria.	transcription
79198	4	335809	6	NULL	NULL	0	NULL	p73	GP		induces					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_122	14634023	p73 induces Bax translocation from cytosol to mitochondria.	transcription
58683	1	335810	5	NULL	NULL	0	NULL	p73			regulates		transcriptionaly			Bax					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_262	14634023	p73 transcriptionally regulates both Bax and PUMA.	transcription
58684	2	335810	5	NULL	NULL	0	NULL	p73			regulates		transcriptionaly			PUMA					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_262	14634023	p73 transcriptionally regulates both Bax and PUMA.	transcription
79199	1	335810	6	NULL	NULL	0	NULL	p73	GP		regulates					Bax	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_262	14634023	p73 transcriptionally regulates both Bax and PUMA.	transcription
79200	2	335810	6	NULL	NULL	0	NULL	p73	GP		regulates					PUMA	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_262	14634023	p73 transcriptionally regulates both Bax and PUMA.	transcription
58685	1	335811	5	NULL	NULL	0	NULL	p73			induce		strongly			Bax				promoter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_269	10207112	It is possible that the induction of the Bax promoter by p73 is via a synergism between p73 and another putative transcription factor also binding to the Bax promoter, which also might explain the strong induction of the Bax promoter by p73.	transcription
58690	1	335812	5	NULL	NULL	0	NULL	PIAS-1			mediates					p73		sumoylation of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_24_10593_s_6	15572666	PIAS-1-mediated sumoylation decreases p73 transcriptional activity on several target promoters, such as Bax. p73 is colocalized in the nucleus with PIAS-1, and sumoylated p73 is located exclusively in the nuclear matrix.	transcription
58691	2	335812	5	NULL	NULL	0	NULL	p73			activates		transcriptionaly			Bax				promoter	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_24_10593_s_6	15572666	PIAS-1-mediated sumoylation decreases p73 transcriptional activity on several target promoters, such as Bax. p73 is colocalized in the nucleus with PIAS-1, and sumoylated p73 is located exclusively in the nuclear matrix.	transcription
58692	3	335812	5	NULL	NULL	0	NULL	statement 1			decreases					statement 2					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_24_10593_s_6	15572666	PIAS-1-mediated sumoylation decreases p73 transcriptional activity on several target promoters, such as Bax. p73 is colocalized in the nucleus with PIAS-1, and sumoylated p73 is located exclusively in the nuclear matrix.	transcription
58693	4	335812	5	NULL	NULL	0	NULL	p73			colocalize with					PIAS-1					NULL	nucleus	0	NULL	NULL	NULL	gw70_molcellbiol_24_24_10593_s_6	15572666	PIAS-1-mediated sumoylation decreases p73 transcriptional activity on several target promoters, such as Bax. p73 is colocalized in the nucleus with PIAS-1, and sumoylated p73 is located exclusively in the nuclear matrix.	transcription
58694	5	335812	5	NULL	NULL	0	NULL	p73		sumoylated	is located in		exclusively			nuclear matrix					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_24_10593_s_6	15572666	PIAS-1-mediated sumoylation decreases p73 transcriptional activity on several target promoters, such as Bax. p73 is colocalized in the nucleus with PIAS-1, and sumoylated p73 is located exclusively in the nuclear matrix.	transcription
79201	1	335812	6	NULL	NULL	0	NULL	PIAS-1	GP		mediates					sumoylation	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_24_10593_s_6	15572666	PIAS-1-mediated sumoylation decreases p73 transcriptional activity on several target promoters, such as Bax. p73 is colocalized in the nucleus with PIAS-1, and sumoylated p73 is located exclusively in the nuclear matrix.	transcription
79202	2	335812	6	NULL	NULL	0	NULL	statement 1	Process		decreases					p73	GP	transcriptional activity of 			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_24_10593_s_6	15572666	PIAS-1-mediated sumoylation decreases p73 transcriptional activity on several target promoters, such as Bax. p73 is colocalized in the nucleus with PIAS-1, and sumoylated p73 is located exclusively in the nuclear matrix.	transcription
79203	3	335812	6	NULL	NULL	0	NULL	p73	GP		is localized in					nucleus	CellComponent				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_24_10593_s_6	15572666	PIAS-1-mediated sumoylation decreases p73 transcriptional activity on several target promoters, such as Bax. p73 is colocalized in the nucleus with PIAS-1, and sumoylated p73 is located exclusively in the nuclear matrix.	transcription
79204	4	335812	6	NULL	NULL	0	NULL	PIAS-1	GP		is localized in					nucleus	CellComponent				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_24_10593_s_6	15572666	PIAS-1-mediated sumoylation decreases p73 transcriptional activity on several target promoters, such as Bax. p73 is colocalized in the nucleus with PIAS-1, and sumoylated p73 is located exclusively in the nuclear matrix.	transcription
79205	5	335812	6	NULL	NULL	0	NULL	p73	GP	sumoylated	is localized in					nuclear matrix	CellComponent				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_24_10593_s_6	15572666	PIAS-1-mediated sumoylation decreases p73 transcriptional activity on several target promoters, such as Bax. p73 is colocalized in the nucleus with PIAS-1, and sumoylated p73 is located exclusively in the nuclear matrix.	transcription
58686	1	335813	5	NULL	NULL	0	NULL	Bax			is translocated to					mitochondria					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_1	14634023	p73 Induces apoptosis via PUMA transactivation and Bax mitochondrial translocation.	transcription
58687	2	335813	5	NULL	NULL	0	NULL	p73			induce					apoptosis					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_1	14634023	p73 Induces apoptosis via PUMA transactivation and Bax mitochondrial translocation.	transcription
58688	3	335813	5	NULL	NULL	0	NULL	statement 2			via					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_1	14634023	p73 Induces apoptosis via PUMA transactivation and Bax mitochondrial translocation.	transcription
58689	4	335813	5	NULL	NULL	0	NULL	statement 2			via					PUMA		transactivation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_1	14634023	p73 Induces apoptosis via PUMA transactivation and Bax mitochondrial translocation.	transcription
79206	1	335813	6	NULL	NULL	0	NULL	p73	GP		induces					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_1	14634023	p73 Induces apoptosis via PUMA transactivation and Bax mitochondrial translocation.	transcription
79207	2	335813	6	NULL	NULL	0	NULL	statement 1	Process		occurs via					PUMA	GP	transactivation of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_1	14634023	p73 Induces apoptosis via PUMA transactivation and Bax mitochondrial translocation.	transcription
79208	3	335813	6	NULL	NULL	0	NULL	Bax	GP		is translocated to					mitochondria	CellComponent				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_1	14634023	p73 Induces apoptosis via PUMA transactivation and Bax mitochondrial translocation.	transcription
79209	4	335813	6	NULL	NULL	0	NULL	statement 1	Process		occurs via					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_1	14634023	p73 Induces apoptosis via PUMA transactivation and Bax mitochondrial translocation.	transcription
58695	1	335814	5	NULL	NULL	0	NULL	Bax			is translocated to					mitochondria					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_151	14634023	These results indicate that p73 induces the mitochondrial translocation of Bax through indirect mechanisms.	transcription
58696	2	335814	5	NULL	NULL	0	NULL	p73			induce		indirectly			statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_151	14634023	These results indicate that p73 induces the mitochondrial translocation of Bax through indirect mechanisms.	transcription
79210	1	335814	6	NULL	NULL	0	NULL	Bax	GP		is translocated to					mitochondria	CellComponent				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_151	14634023	These results indicate that p73 induces the mitochondrial translocation of Bax through indirect mechanisms.	transcription
79211	2	335814	6	NULL	NULL	0	NULL	p73	GP		induces					statement 1	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_151	14634023	These results indicate that p73 induces the mitochondrial translocation of Bax through indirect mechanisms.	transcription
58697	1	335815	5	NULL	NULL	0	NULL	Bax			is translocated to					mitochondria					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_260	14634023	p73 induces apoptosis via PUMA-mediated Bax mitochondrial translocation.	transcription
58698	2	335815	5	NULL	NULL	0	NULL	PUMA			mediates					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_260	14634023	p73 induces apoptosis via PUMA-mediated Bax mitochondrial translocation.	transcription
58699	3	335815	5	NULL	NULL	0	NULL	p73			induce					apoptosis					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_260	14634023	p73 induces apoptosis via PUMA-mediated Bax mitochondrial translocation.	transcription
58700	4	335815	5	NULL	NULL	0	NULL	statement 3			via					statement 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_260	14634023	p73 induces apoptosis via PUMA-mediated Bax mitochondrial translocation.	transcription
79212	1	335815	6	NULL	NULL	0	NULL	Bax	GP		is translocated to					mitochondria	CellComponent				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_260	14634023	p73 induces apoptosis via PUMA-mediated Bax mitochondrial translocation.	transcription
79213	2	335815	6	NULL	NULL	0	NULL	PUMA	Chemical		mediates					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_260	14634023	p73 induces apoptosis via PUMA-mediated Bax mitochondrial translocation.	transcription
79214	3	335815	6	NULL	NULL	0	NULL	p73	GP		induces					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_260	14634023	p73 induces apoptosis via PUMA-mediated Bax mitochondrial translocation.	transcription
79215	4	335815	6	NULL	NULL	0	NULL	statement 3	Process		occurs via					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_260	14634023	p73 induces apoptosis via PUMA-mediated Bax mitochondrial translocation.	transcription
79216	1	335816	6	NULL	NULL	0	NULL	Bax	GP		activates					transcription	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_14_10202_s_354	10744705	WT1 represses p73- and p53-dependent transcription activation from the  bax and the  mdm2 promoters.	transcription
79217	2	335816	6	NULL	NULL	0	NULL	statement 1	Process		is dependent on					p73	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_14_10202_s_354	10744705	WT1 represses p73- and p53-dependent transcription activation from the  bax and the  mdm2 promoters.	transcription
79218	3	335816	6	NULL	NULL	0	NULL	WT1	GP		represses					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_14_10202_s_354	10744705	WT1 represses p73- and p53-dependent transcription activation from the  bax and the  mdm2 promoters.	transcription
79219	4	335816	6	NULL	NULL	0	NULL	mdm2	GP		activates					transcription	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_14_10202_s_354	10744705	WT1 represses p73- and p53-dependent transcription activation from the  bax and the  mdm2 promoters.	transcription
79220	5	335816	6	NULL	NULL	0	NULL	statement 4	Process		is dependent on					p53	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_14_10202_s_354	10744705	WT1 represses p73- and p53-dependent transcription activation from the  bax and the  mdm2 promoters.	transcription
79221	6	335816	6	NULL	NULL	0	NULL	WT1	GP		represses					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_14_10202_s_354	10744705	WT1 represses p73- and p53-dependent transcription activation from the  bax and the  mdm2 promoters.	transcription
58701	1	335817	5	NULL	NULL	0	NULL	Bax			is translocated from					cytosol					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_112	14634023	p73 Indirectly Induces Bax Mitochondrial Relocalization --  Bax translocation from cytosol to mitochondria is a critical step in p53-mediated apoptosis ( ).	transcription
58702	2	335817	5	NULL	NULL	0	NULL	Bax			is translocated to					mitochondria					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_112	14634023	p73 Indirectly Induces Bax Mitochondrial Relocalization --  Bax translocation from cytosol to mitochondria is a critical step in p53-mediated apoptosis ( ).	transcription
58703	3	335817	5	NULL	NULL	0	NULL	statement 1			occurs simultaneously with					statement 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_112	14634023	p73 Indirectly Induces Bax Mitochondrial Relocalization --  Bax translocation from cytosol to mitochondria is a critical step in p53-mediated apoptosis ( ).	transcription
58704	4	335817	5	NULL	NULL	0	NULL	p53			mediates					apoptosis					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_112	14634023	p73 Indirectly Induces Bax Mitochondrial Relocalization --  Bax translocation from cytosol to mitochondria is a critical step in p53-mediated apoptosis ( ).	transcription
58705	5	335817	5	NULL	NULL	0	NULL	statement 3			is critical for					statement 4					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_112	14634023	p73 Indirectly Induces Bax Mitochondrial Relocalization --  Bax translocation from cytosol to mitochondria is a critical step in p53-mediated apoptosis ( ).	transcription
58706	6	335817	5	NULL	NULL	0	NULL	p73			induce		indirectly			statement 3					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_112	14634023	p73 Indirectly Induces Bax Mitochondrial Relocalization --  Bax translocation from cytosol to mitochondria is a critical step in p53-mediated apoptosis ( ).	transcription
79222	1	335817	6	NULL	NULL	0	NULL	Bax	GP		is translocated to					mitochondria	CellComponent				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_112	14634023	p73 Indirectly Induces Bax Mitochondrial Relocalization --  Bax translocation from cytosol to mitochondria is a critical step in p53-mediated apoptosis ( ).	transcription
79223	2	335817	6	NULL	NULL	0	NULL	Bax	GP		is translocated from					cytosol	CellComponent				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_112	14634023	p73 Indirectly Induces Bax Mitochondrial Relocalization --  Bax translocation from cytosol to mitochondria is a critical step in p53-mediated apoptosis ( ).	transcription
79224	3	335817	6	NULL	NULL	0	NULL	statement 1	Process		occurs simultaneously with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_112	14634023	p73 Indirectly Induces Bax Mitochondrial Relocalization --  Bax translocation from cytosol to mitochondria is a critical step in p53-mediated apoptosis ( ).	transcription
79225	4	335817	6	NULL	NULL	0	NULL	p73	GP		induces					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_112	14634023	p73 Indirectly Induces Bax Mitochondrial Relocalization --  Bax translocation from cytosol to mitochondria is a critical step in p53-mediated apoptosis ( ).	transcription
58707	1	335819	5	NULL	NULL	0	NULL	p53 virus		infection of	induce					p21		expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2951_s_195	11706030	Apparently, expression of p21 and Bax was induced by infection of the p53 and p73 viruses (Fig.  6,  A and  B,  p21 and  Bax panels,  lanes 1 and  2).	transcription
58708	2	335819	5	NULL	NULL	0	NULL	p73 virus		infection of	induce					p21		expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2951_s_195	11706030	Apparently, expression of p21 and Bax was induced by infection of the p53 and p73 viruses (Fig.  6,  A and  B,  p21 and  Bax panels,  lanes 1 and  2).	transcription
58709	3	335819	5	NULL	NULL	0	NULL	p73 virus		infection of	induce					Bax		expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2951_s_195	11706030	Apparently, expression of p21 and Bax was induced by infection of the p53 and p73 viruses (Fig.  6,  A and  B,  p21 and  Bax panels,  lanes 1 and  2).	transcription
58710	4	335819	5	NULL	NULL	0	NULL	p53 virus		infection of	induce					Bax		expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2951_s_195	11706030	Apparently, expression of p21 and Bax was induced by infection of the p53 and p73 viruses (Fig.  6,  A and  B,  p21 and  Bax panels,  lanes 1 and  2).	transcription
79226	1	335819	6	NULL	NULL	0	NULL	p53	GP		induces					p21	GP	expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2951_s_195	11706030	Apparently, expression of p21 and Bax was induced by infection of the p53 and p73 viruses (Fig.  6,  A and  B,  p21 and  Bax panels,  lanes 1 and  2).	transcription
79227	2	335819	6	NULL	NULL	0	NULL	p73	GP		induces					Bax	GP	expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2951_s_195	11706030	Apparently, expression of p21 and Bax was induced by infection of the p53 and p73 viruses (Fig.  6,  A and  B,  p21 and  Bax panels,  lanes 1 and  2).	transcription
58711	1	335820	5	NULL	NULL	0	NULL	p73			cooperates with					p53					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_7_5945_s_21	15572378	p73 cooperates with p53 to induce specific targets such as PERP, Bax, and Noxa, which are involved in the p53-mediated induction of apoptosis.	transcription
58712	2	335820	5	NULL	NULL	0	NULL	statement 1			induce					PERP					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_7_5945_s_21	15572378	p73 cooperates with p53 to induce specific targets such as PERP, Bax, and Noxa, which are involved in the p53-mediated induction of apoptosis.	transcription
58713	3	335820	5	NULL	NULL	0	NULL	statement 1			induce					Bax					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_7_5945_s_21	15572378	p73 cooperates with p53 to induce specific targets such as PERP, Bax, and Noxa, which are involved in the p53-mediated induction of apoptosis.	transcription
58714	4	335820	5	NULL	NULL	0	NULL	statement 1			induce					Noxa					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_7_5945_s_21	15572378	p73 cooperates with p53 to induce specific targets such as PERP, Bax, and Noxa, which are involved in the p53-mediated induction of apoptosis.	transcription
58715	5	335820	5	NULL	NULL	0	NULL	p53			induce					apoptosis					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_7_5945_s_21	15572378	p73 cooperates with p53 to induce specific targets such as PERP, Bax, and Noxa, which are involved in the p53-mediated induction of apoptosis.	transcription
58716	6	335820	5	NULL	NULL	0	NULL	PERP			is involved in					statement 5					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_7_5945_s_21	15572378	p73 cooperates with p53 to induce specific targets such as PERP, Bax, and Noxa, which are involved in the p53-mediated induction of apoptosis.	transcription
58717	7	335820	5	NULL	NULL	0	NULL	Bax			is involved in					statement 5					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_7_5945_s_21	15572378	p73 cooperates with p53 to induce specific targets such as PERP, Bax, and Noxa, which are involved in the p53-mediated induction of apoptosis.	transcription
58718	8	335820	5	NULL	NULL	0	NULL	Noxa			is involved in					statement 5					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_7_5945_s_21	15572378	p73 cooperates with p53 to induce specific targets such as PERP, Bax, and Noxa, which are involved in the p53-mediated induction of apoptosis.	transcription
79228	1	335820	6	NULL	NULL	0	NULL	p53	GP		mediates					apoptosis	Process	induction of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_7_5945_s_21	15572378	p73 cooperates with p53 to induce specific targets such as PERP, Bax, and Noxa, which are involved in the p53-mediated induction of apoptosis.	transcription
79229	2	335820	6	NULL	NULL	0	NULL	PERP	GP		is involved in					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_7_5945_s_21	15572378	p73 cooperates with p53 to induce specific targets such as PERP, Bax, and Noxa, which are involved in the p53-mediated induction of apoptosis.	transcription
79230	3	335820	6	NULL	NULL	0	NULL	Bax	GP		is involved in					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_7_5945_s_21	15572378	p73 cooperates with p53 to induce specific targets such as PERP, Bax, and Noxa, which are involved in the p53-mediated induction of apoptosis.	transcription
79231	4	335820	6	NULL	NULL	0	NULL	Noxa	GP		is involved in					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_7_5945_s_21	15572378	p73 cooperates with p53 to induce specific targets such as PERP, Bax, and Noxa, which are involved in the p53-mediated induction of apoptosis.	transcription
58719	1	335821	5	NULL	NULL	0	NULL	Bax			is apoptotic target of					p53					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_7_5945_s_364	15572378	Exogenous expression of both p53 and p73 in Saos-2 cells resulted in the activation of p53 apoptotic target Bax ( Fig. 9 A).	transcription
58720	2	335821	5	NULL	NULL	0	NULL	p53		exogenous expression of	activates					statement 1					NULL	Saos-2 cells	0	NULL	NULL	NULL	gw70_jbiolchem_280_7_5945_s_364	15572378	Exogenous expression of both p53 and p73 in Saos-2 cells resulted in the activation of p53 apoptotic target Bax ( Fig. 9 A).	transcription
58721	3	335821	5	NULL	NULL	0	NULL	p73		exogenous expression of	activates					statement 1					NULL	Saos-2 cells	0	NULL	NULL	NULL	gw70_jbiolchem_280_7_5945_s_364	15572378	Exogenous expression of both p53 and p73 in Saos-2 cells resulted in the activation of p53 apoptotic target Bax ( Fig. 9 A).	transcription
79232	1	335821	6	NULL	NULL	0	NULL	p53	GP	expression of	results in					Bax	GP	activation of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_7_5945_s_364	15572378	Exogenous expression of both p53 and p73 in Saos-2 cells resulted in the activation of p53 apoptotic target Bax ( Fig. 9 A).	transcription
79233	2	335821	6	NULL	NULL	0	NULL	p73	GP	expression of	results in					Bax	GP	activation of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_7_5945_s_364	15572378	Exogenous expression of both p53 and p73 in Saos-2 cells resulted in the activation of p53 apoptotic target Bax ( Fig. 9 A).	transcription
58722	1	335822	5	NULL	NULL	0	NULL	p73 isoforms		overexpression of	promotes					cell death					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_5	14634023	Overexpression of p73 isoforms promotes cell death and  bax promoter transactivation in a time-dependent manner.	transcription
58723	2	335822	5	NULL	NULL	0	NULL	p73 isoforms		overexpression of	transactivates					Bax				promoter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_5	14634023	Overexpression of p73 isoforms promotes cell death and  bax promoter transactivation in a time-dependent manner.	transcription
79234	1	335822	6	NULL	NULL	0	NULL	p73 isoforms	GP	overexpression of	promotes					cell death	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_5	14634023	Overexpression of p73 isoforms promotes cell death and  bax promoter transactivation in a time-dependent manner.	transcription
79235	2	335822	6	NULL	NULL	0	NULL	p73 isoforms	GP	overexpression of	results in					Bax 	GP	transactivation of 		promoter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_5	14634023	Overexpression of p73 isoforms promotes cell death and  bax promoter transactivation in a time-dependent manner.	transcription
58724	1	335823	5	NULL	NULL	0	NULL	Bax		translocation of	is induced by		may;;directly			p73 protein					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_139	14634023	At the same time, the experiment would elucidate if Bax translocation is directly induced by the p73 protein  per se.	transcription
58725	1	335824	5	NULL	NULL	0	NULL	bax-Pruc		transactivation of	is dependent on					p73					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_214	14634023	The results show that delta84p73beta strongly inhibited both p73- and p53-dependent transactivation of the  bax-Pruc ( Fig. 7 A).	transcription
58726	2	335824	5	NULL	NULL	0	NULL	bax-Pruc		transactivation of	is dependent on					p53					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_214	14634023	The results show that delta84p73beta strongly inhibited both p73- and p53-dependent transactivation of the  bax-Pruc ( Fig. 7 A).	transcription
58727	3	335824	5	NULL	NULL	0	NULL	delta84p73beta			inhibits		strongly			statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_214	14634023	The results show that delta84p73beta strongly inhibited both p73- and p53-dependent transactivation of the  bax-Pruc ( Fig. 7 A).	transcription
58728	4	335824	5	NULL	NULL	0	NULL	delta84p73beta			inhibits		strongly			statement 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_214	14634023	The results show that delta84p73beta strongly inhibited both p73- and p53-dependent transactivation of the  bax-Pruc ( Fig. 7 A).	transcription
79236	1	335824	6	NULL	NULL	0	NULL	p73	GP		transactivates					Bax-Prunc	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_214	14634023	The results show that delta84p73beta strongly inhibited both p73- and p53-dependent transactivation of the  bax-Pruc ( Fig. 7 A).	transcription
79237	2	335824	6	NULL	NULL	0	NULL	p53	GP		transactivates					Bax-Prunc	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_214	14634023	The results show that delta84p73beta strongly inhibited both p73- and p53-dependent transactivation of the  bax-Pruc ( Fig. 7 A).	transcription
79238	3	335824	6	NULL	NULL	0	NULL	delta84p73beta	GP		inhibits		strongly			statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_214	14634023	The results show that delta84p73beta strongly inhibited both p73- and p53-dependent transactivation of the  bax-Pruc ( Fig. 7 A).	transcription
79239	4	335824	6	NULL	NULL	0	NULL	delta84p73beta	GP		inhibits		strongly			statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_214	14634023	The results show that delta84p73beta strongly inhibited both p73- and p53-dependent transactivation of the  bax-Pruc ( Fig. 7 A).	transcription
58729	1	335825	5	NULL	NULL	0	NULL	deltaNp73			does not activate					transcription					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_236	14634023	As shown in  Fig. 7 B, deltaNp73 did not have transcriptional activity but efficiently inhibited p73- and p53-dependent transactivation of  bax-PrLuc.	transcription
58730	2	335825	5	NULL	NULL	0	NULL	bax-PrLuc		transactivation of	is dependent on					p53					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_236	14634023	As shown in  Fig. 7 B, deltaNp73 did not have transcriptional activity but efficiently inhibited p73- and p53-dependent transactivation of  bax-PrLuc.	transcription
58731	3	335825	5	NULL	NULL	0	NULL	bax-PrLuc		transactivation of	is dependent on					p73					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_236	14634023	As shown in  Fig. 7 B, deltaNp73 did not have transcriptional activity but efficiently inhibited p73- and p53-dependent transactivation of  bax-PrLuc.	transcription
58732	4	335825	5	NULL	NULL	0	NULL	deltaNp73			inhibit		efficiently			statement 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_236	14634023	As shown in  Fig. 7 B, deltaNp73 did not have transcriptional activity but efficiently inhibited p73- and p53-dependent transactivation of  bax-PrLuc.	transcription
58733	5	335825	5	NULL	NULL	0	NULL	deltaNp73			inhibit		efficiently			statement 3					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_236	14634023	As shown in  Fig. 7 B, deltaNp73 did not have transcriptional activity but efficiently inhibited p73- and p53-dependent transactivation of  bax-PrLuc.	transcription
58734	1	335826	5	NULL	NULL	0	NULL	p73			induce					cell death					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_249	14634023	Therefore, p73-induced cell death cannot rely only on the ability of p73 to up-regulate  bax expression.	transcription
58735	2	335826	5	NULL	NULL	0	NULL	p73			up-regulates					bax		expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_249	14634023	Therefore, p73-induced cell death cannot rely only on the ability of p73 to up-regulate  bax expression.	transcription
58736	3	335826	5	NULL	NULL	0	NULL	statement 1			does not rely on					statement 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_249	14634023	Therefore, p73-induced cell death cannot rely only on the ability of p73 to up-regulate  bax expression.	transcription
79240	1	335826	6	NULL	NULL	0	NULL	p73	GP		up-regulates					bax	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_249	14634023	Therefore, p73-induced cell death cannot rely only on the ability of p73 to up-regulate  bax expression.	transcription
58737	1	335827	5	NULL	NULL	0	NULL	p53			regulates					BAX					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_4_2249_s_20	12427762	For example, p73 induces p53-regulated  BAX in A2870 ovarian cells but not in H1229 lung cancer cells ( ,  ).	transcription
58738	2	335827	5	NULL	NULL	0	NULL	p73			induces					statement 1					NULL	A2870 ovarian cells	0	NULL	NULL	NULL	gw70_jbiolchem_278_4_2249_s_20	12427762	For example, p73 induces p53-regulated  BAX in A2870 ovarian cells but not in H1229 lung cancer cells ( ,  ).	transcription
58739	3	335827	5	NULL	NULL	0	NULL	p73			does not induce					statement 1					NULL	H1229 lung cancer cells	0	NULL	NULL	NULL	gw70_jbiolchem_278_4_2249_s_20	12427762	For example, p73 induces p53-regulated  BAX in A2870 ovarian cells but not in H1229 lung cancer cells ( ,  ).	transcription
79241	1	335827	6	NULL	NULL	0	NULL	p53	GP		regulates					BAX	GP				NULL	A2870 ovarian cells	0	NULL	NULL	NULL	gw70_jbiolchem_278_4_2249_s_20	12427762	For example, p73 induces p53-regulated  BAX in A2870 ovarian cells but not in H1229 lung cancer cells ( ,  ).	transcription
79242	2	335827	6	NULL	NULL	0	NULL	p73	GP		induces					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_4_2249_s_20	12427762	For example, p73 induces p53-regulated  BAX in A2870 ovarian cells but not in H1229 lung cancer cells ( ,  ).	transcription
79243	3	335827	6	NULL	NULL	0	NULL	p73	GP		does not induce					statement 1	Process				NULL	H1229 lung cancer cells	0	NULL	NULL	NULL	gw70_jbiolchem_278_4_2249_s_20	12427762	For example, p73 induces p53-regulated  BAX in A2870 ovarian cells but not in H1229 lung cancer cells ( ,  ).	transcription
58740	1	335828	5	NULL	NULL	0	NULL	apoptosis			is dependent on					p53					NULL		0	NULL	NULL	NULL	gw60_cancercell_1_4_311_s_28	12086844	Remarkably, however, loss of p63 and p73 severely affected the induction of  bax and  PERP, two genes thought to mediate p53-dependent apoptosis.	transcription
58741	2	335828	5	NULL	NULL	0	NULL	bax gene			mediates					statement 1					NULL		0	NULL	NULL	NULL	gw60_cancercell_1_4_311_s_28	12086844	Remarkably, however, loss of p63 and p73 severely affected the induction of  bax and  PERP, two genes thought to mediate p53-dependent apoptosis.	transcription
58742	3	335828	5	NULL	NULL	0	NULL	PERP gene			mediates					statement 1					NULL		0	NULL	NULL	NULL	gw60_cancercell_1_4_311_s_28	12086844	Remarkably, however, loss of p63 and p73 severely affected the induction of  bax and  PERP, two genes thought to mediate p53-dependent apoptosis.	transcription
58743	4	335828	5	NULL	NULL	0	NULL	p63		loss of	affects		severely			bax gene		induction of			NULL		0	NULL	NULL	NULL	gw60_cancercell_1_4_311_s_28	12086844	Remarkably, however, loss of p63 and p73 severely affected the induction of  bax and  PERP, two genes thought to mediate p53-dependent apoptosis.	transcription
58744	5	335828	5	NULL	NULL	0	NULL	p63		loss of	affects		severely			PERP gene		induction of			NULL		NULL	NULL	NULL	NULL	gw60_cancercell_1_4_311_s_28	12086844	Remarkably, however, loss of p63 and p73 severely affected the induction of  bax and  PERP, two genes thought to mediate p53-dependent apoptosis.	transcription
58745	6	335828	5	NULL	NULL	0	NULL	p73		loss of	affects		severely			bax gene		induction of			NULL		0	NULL	NULL	NULL	gw60_cancercell_1_4_311_s_28	12086844	Remarkably, however, loss of p63 and p73 severely affected the induction of  bax and  PERP, two genes thought to mediate p53-dependent apoptosis.	transcription
58746	7	335828	5	NULL	NULL	0	NULL	p73		loss of	affects		severely			PERP gene		induction of			NULL		NULL	NULL	NULL	NULL	gw60_cancercell_1_4_311_s_28	12086844	Remarkably, however, loss of p63 and p73 severely affected the induction of  bax and  PERP, two genes thought to mediate p53-dependent apoptosis.	transcription
58747	1	335829	5	NULL	NULL	0	NULL	p21			is a type of					p53 target gene					NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_2_513_s_17	10606650	p73 can transcriptionally activate p53 target genes such as p21 or BAX and induces apoptosis in p53-null Saos-2 cells ( 12, 13).	transcription
58748	2	335829	5	NULL	NULL	0	NULL	BAX			is a type of					p53 target gene					NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_2_513_s_17	10606650	p73 can transcriptionally activate p53 target genes such as p21 or BAX and induces apoptosis in p53-null Saos-2 cells ( 12, 13).	transcription
58749	3	335829	5	NULL	NULL	0	NULL	p73			activates		transcriptionaly			p21 gene					NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_2_513_s_17	10606650	p73 can transcriptionally activate p53 target genes such as p21 or BAX and induces apoptosis in p53-null Saos-2 cells ( 12, 13).	transcription
58750	4	335829	5	NULL	NULL	0	NULL	p73			activates		transcriptionaly			BAX gene					NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_2_513_s_17	10606650	p73 can transcriptionally activate p53 target genes such as p21 or BAX and induces apoptosis in p53-null Saos-2 cells ( 12, 13).	transcription
58751	5	335829	5	NULL	NULL	0	NULL	p73			induces					apoptosis					NULL	p53-null Saos-2 cells	0	NULL	NULL	NULL	gw60_nucleicacidsres_28_2_513_s_17	10606650	p73 can transcriptionally activate p53 target genes such as p21 or BAX and induces apoptosis in p53-null Saos-2 cells ( 12, 13).	transcription
79244	1	335829	6	NULL	NULL	0	NULL	p73	GP		activates					p21	GP				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_2_513_s_17	10606650	p73 can transcriptionally activate p53 target genes such as p21 or BAX and induces apoptosis in p53-null Saos-2 cells ( 12, 13).	transcription
79245	2	335829	6	NULL	NULL	0	NULL	p73	GP		activates					BAX	GP				NULL		0	NULL	NULL	NULL	gw60_nucleicacidsres_28_2_513_s_17	10606650	p73 can transcriptionally activate p53 target genes such as p21 or BAX and induces apoptosis in p53-null Saos-2 cells ( 12, 13).	transcription
79246	3	335829	6	NULL	NULL	0	NULL	p73	GP		induces					apoptosis	Process				NULL	p53-null Saos-2 cells	0	NULL	NULL	NULL	gw60_nucleicacidsres_28_2_513_s_17	10606650	p73 can transcriptionally activate p53 target genes such as p21 or BAX and induces apoptosis in p53-null Saos-2 cells ( 12, 13).	transcription
58752	1	335830	5	NULL	NULL	0	NULL	ik3-1		co-infection of	does not alter		significantly			p53		expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2951_s_201	11706030	Co-infection of ik3-1 or ik3-1-deltaC does not significantly alter expression of p53, p73, p21, or Bax.	transcription
58753	2	335830	5	NULL	NULL	0	NULL	ik3-1		co-infection of	does not alter		significantly			p73		expression of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2951_s_201	11706030	Co-infection of ik3-1 or ik3-1-deltaC does not significantly alter expression of p53, p73, p21, or Bax.	transcription
58754	3	335830	5	NULL	NULL	0	NULL	ik3-1		co-infection of	does not alter		significantly			p21		expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2951_s_201	11706030	Co-infection of ik3-1 or ik3-1-deltaC does not significantly alter expression of p53, p73, p21, or Bax.	transcription
58755	4	335830	5	NULL	NULL	0	NULL	ik3-1		co-infection of	does not alter		significantly			Bax		expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2951_s_201	11706030	Co-infection of ik3-1 or ik3-1-deltaC does not significantly alter expression of p53, p73, p21, or Bax.	transcription
58756	5	335830	5	NULL	NULL	0	NULL	ik3-1-deltaC		co-infection of	does not alter		significantly			p53		expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2951_s_201	11706030	Co-infection of ik3-1 or ik3-1-deltaC does not significantly alter expression of p53, p73, p21, or Bax.	transcription
58757	6	335830	5	NULL	NULL	0	NULL	ik3-1-deltaC		co-infection of	does not alter		significantly			p73		expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2951_s_201	11706030	Co-infection of ik3-1 or ik3-1-deltaC does not significantly alter expression of p53, p73, p21, or Bax.	transcription
58758	7	335830	5	NULL	NULL	0	NULL	ik3-1-deltaC		co-infection of	does not alter		significantly			p21		expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2951_s_201	11706030	Co-infection of ik3-1 or ik3-1-deltaC does not significantly alter expression of p53, p73, p21, or Bax.	transcription
58759	8	335830	5	NULL	NULL	0	NULL	ik3-1-deltaC		co-infection of	does not alter		significantly			Bax		expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2951_s_201	11706030	Co-infection of ik3-1 or ik3-1-deltaC does not significantly alter expression of p53, p73, p21, or Bax.	transcription
58760	1	335831	5	NULL	NULL	0	NULL	p73			is a homolog of					p53					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_47_33747_s_251	10559267	The p53 homolog p73 does not selectively inhibit the ability of p53 to activate transcription through the  bax promoter.	transcription
58761	2	335831	5	NULL	NULL	0	NULL	p53			activates					transcription					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_47_33747_s_251	10559267	The p53 homolog p73 does not selectively inhibit the ability of p53 to activate transcription through the  bax promoter.	transcription
58762	3	335831	5	NULL	NULL	0	NULL	statement 2			through					bax				promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_47_33747_s_251	10559267	The p53 homolog p73 does not selectively inhibit the ability of p53 to activate transcription through the  bax promoter.	transcription
58763	4	335831	5	NULL	NULL	0	NULL	p73			does not inhibit		selectively			statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_47_33747_s_251	10559267	The p53 homolog p73 does not selectively inhibit the ability of p53 to activate transcription through the  bax promoter.	transcription
79257	1	335831	6	NULL	NULL	0	NULL	p53	GP		transactivates					bax	GP			promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_47_33747_s_251	10559267	The p53 homolog p73 does not selectively inhibit the ability of p53 to activate transcription through the  bax promoter.	transcription
79258	2	335831	6	NULL	NULL	0	NULL	p73	GP		does not inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_47_33747_s_251	10559267	The p53 homolog p73 does not selectively inhibit the ability of p53 to activate transcription through the  bax promoter.	transcription
58764	1	335832	5	NULL	NULL	0	NULL	p63		loss of	affects		severely			bax gene		induction of			NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_25_6_857_s_68	15033906	While induction of  p21 and  MDM2 occurred normally in p63 - / - , p73 - / - , and double-null E1A-expressing MEFs, loss of p63 and p73 severely affected the induction of  bax,  NOXA and  PERP, genes thought to mediate p53-dependent apoptosis.	transcription
58765	2	335832	5	NULL	NULL	0	NULL	p63		loss of	affects		severely			NOXA gene		induction of			NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_25_6_857_s_68	15033906	While induction of  p21 and  MDM2 occurred normally in p63 - / - , p73 - / - , and double-null E1A-expressing MEFs, loss of p63 and p73 severely affected the induction of  bax,  NOXA and  PERP, genes thought to mediate p53-dependent apoptosis.	transcription
58766	3	335832	5	NULL	NULL	0	NULL	p63		loss of	affects		severely			PERP gene		induction of			NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_25_6_857_s_68	15033906	While induction of  p21 and  MDM2 occurred normally in p63 - / - , p73 - / - , and double-null E1A-expressing MEFs, loss of p63 and p73 severely affected the induction of  bax,  NOXA and  PERP, genes thought to mediate p53-dependent apoptosis.	transcription
58767	4	335832	5	NULL	NULL	0	NULL	p73 		loss of	affects		severely			bax gene		induction of			NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_25_6_857_s_68	15033906	While induction of  p21 and  MDM2 occurred normally in p63 - / - , p73 - / - , and double-null E1A-expressing MEFs, loss of p63 and p73 severely affected the induction of  bax,  NOXA and  PERP, genes thought to mediate p53-dependent apoptosis.	transcription
58768	5	335832	5	NULL	NULL	0	NULL	p73		loss of	affects		severely			NOXA gene		induction of			NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_25_6_857_s_68	15033906	While induction of  p21 and  MDM2 occurred normally in p63 - / - , p73 - / - , and double-null E1A-expressing MEFs, loss of p63 and p73 severely affected the induction of  bax,  NOXA and  PERP, genes thought to mediate p53-dependent apoptosis.	transcription
58769	6	335832	5	NULL	NULL	0	NULL	p73		loss of	affects		severely			PERP gene		induction of			NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_25_6_857_s_68	15033906	While induction of  p21 and  MDM2 occurred normally in p63 - / - , p73 - / - , and double-null E1A-expressing MEFs, loss of p63 and p73 severely affected the induction of  bax,  NOXA and  PERP, genes thought to mediate p53-dependent apoptosis.	transcription
58770	7	335832	5	NULL	NULL	0	NULL	apoptosis			is dependent on					p53					NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_25_6_857_s_68	15033906	While induction of  p21 and  MDM2 occurred normally in p63 - / - , p73 - / - , and double-null E1A-expressing MEFs, loss of p63 and p73 severely affected the induction of  bax,  NOXA and  PERP, genes thought to mediate p53-dependent apoptosis.	transcription
58771	8	335832	5	NULL	NULL	0	NULL	bax gene			mediates		may			statement 7					NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_25_6_857_s_68	15033906	While induction of  p21 and  MDM2 occurred normally in p63 - / - , p73 - / - , and double-null E1A-expressing MEFs, loss of p63 and p73 severely affected the induction of  bax,  NOXA and  PERP, genes thought to mediate p53-dependent apoptosis.	transcription
58772	9	335832	5	NULL	NULL	0	NULL	NOXA gene			mediates		may			statement 7					NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_25_6_857_s_68	15033906	While induction of  p21 and  MDM2 occurred normally in p63 - / - , p73 - / - , and double-null E1A-expressing MEFs, loss of p63 and p73 severely affected the induction of  bax,  NOXA and  PERP, genes thought to mediate p53-dependent apoptosis.	transcription
58773	10	335832	5	NULL	NULL	0	NULL	PERP gene			mediates		may			statement 7					NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_25_6_857_s_68	15033906	While induction of  p21 and  MDM2 occurred normally in p63 - / - , p73 - / - , and double-null E1A-expressing MEFs, loss of p63 and p73 severely affected the induction of  bax,  NOXA and  PERP, genes thought to mediate p53-dependent apoptosis.	transcription
58774	1	335833	5	NULL	NULL	0	NULL	Bax			is a type of					proapoptotic gene					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1341_s_188	14729977	Since expression of ASPP1 or ASPP2 stimulated the transactivation function of p63 and p73 on promoters of proapoptotic genes, such as Bax, PIG3, and PUMA, it is likely that ASPP1 and ASPP2 also stimulate the apoptotic function of p63 and p73.	transcription
58775	2	335833	5	NULL	NULL	0	NULL	PIG3			is a type of					proapoptotic gene					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1341_s_188	14729977	Since expression of ASPP1 or ASPP2 stimulated the transactivation function of p63 and p73 on promoters of proapoptotic genes, such as Bax, PIG3, and PUMA, it is likely that ASPP1 and ASPP2 also stimulate the apoptotic function of p63 and p73.	transcription
58776	3	335833	5	NULL	NULL	0	NULL	PUMA			is a type of					proapoptotic gene					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1341_s_188	14729977	Since expression of ASPP1 or ASPP2 stimulated the transactivation function of p63 and p73 on promoters of proapoptotic genes, such as Bax, PIG3, and PUMA, it is likely that ASPP1 and ASPP2 also stimulate the apoptotic function of p63 and p73.	transcription
58777	4	335833	5	NULL	NULL	0	NULL	p63			transactivates					Bax				promoter	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1341_s_188	14729977	Since expression of ASPP1 or ASPP2 stimulated the transactivation function of p63 and p73 on promoters of proapoptotic genes, such as Bax, PIG3, and PUMA, it is likely that ASPP1 and ASPP2 also stimulate the apoptotic function of p63 and p73.	transcription
58778	5	335833	5	NULL	NULL	0	NULL	p63			transactivates					PIG3				promoter	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1341_s_188	14729977	Since expression of ASPP1 or ASPP2 stimulated the transactivation function of p63 and p73 on promoters of proapoptotic genes, such as Bax, PIG3, and PUMA, it is likely that ASPP1 and ASPP2 also stimulate the apoptotic function of p63 and p73.	transcription
58779	6	335833	5	NULL	NULL	0	NULL	p63			transactivates					PUMA				promoter	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1341_s_188	14729977	Since expression of ASPP1 or ASPP2 stimulated the transactivation function of p63 and p73 on promoters of proapoptotic genes, such as Bax, PIG3, and PUMA, it is likely that ASPP1 and ASPP2 also stimulate the apoptotic function of p63 and p73.	transcription
58780	7	335833	5	NULL	NULL	0	NULL	p73			transactivates					Bax				promoter	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1341_s_188	14729977	Since expression of ASPP1 or ASPP2 stimulated the transactivation function of p63 and p73 on promoters of proapoptotic genes, such as Bax, PIG3, and PUMA, it is likely that ASPP1 and ASPP2 also stimulate the apoptotic function of p63 and p73.	transcription
58781	8	335833	5	NULL	NULL	0	NULL	p73			transactivates					PIG3				promoter	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1341_s_188	14729977	Since expression of ASPP1 or ASPP2 stimulated the transactivation function of p63 and p73 on promoters of proapoptotic genes, such as Bax, PIG3, and PUMA, it is likely that ASPP1 and ASPP2 also stimulate the apoptotic function of p63 and p73.	transcription
58782	9	335833	5	NULL	NULL	0	NULL	p73			transactivates					PUMA				promoter	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1341_s_188	14729977	Since expression of ASPP1 or ASPP2 stimulated the transactivation function of p63 and p73 on promoters of proapoptotic genes, such as Bax, PIG3, and PUMA, it is likely that ASPP1 and ASPP2 also stimulate the apoptotic function of p63 and p73.	transcription
58783	10	335833	5	NULL	NULL	0	NULL	ASPP1			stimulates					statement 4					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1341_s_188	14729977	Since expression of ASPP1 or ASPP2 stimulated the transactivation function of p63 and p73 on promoters of proapoptotic genes, such as Bax, PIG3, and PUMA, it is likely that ASPP1 and ASPP2 also stimulate the apoptotic function of p63 and p73.	transcription
58784	11	335833	5	NULL	NULL	0	NULL	ASPP1			stimulates					statement 5					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1341_s_188	14729977	Since expression of ASPP1 or ASPP2 stimulated the transactivation function of p63 and p73 on promoters of proapoptotic genes, such as Bax, PIG3, and PUMA, it is likely that ASPP1 and ASPP2 also stimulate the apoptotic function of p63 and p73.	transcription
58785	12	335833	5	NULL	NULL	0	NULL	ASPP1			stimulates					statement 6					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1341_s_188	14729977	Since expression of ASPP1 or ASPP2 stimulated the transactivation function of p63 and p73 on promoters of proapoptotic genes, such as Bax, PIG3, and PUMA, it is likely that ASPP1 and ASPP2 also stimulate the apoptotic function of p63 and p73.	transcription
58786	13	335833	5	NULL	NULL	0	NULL	ASPP1			stimulates					statement 7					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1341_s_188	14729977	Since expression of ASPP1 or ASPP2 stimulated the transactivation function of p63 and p73 on promoters of proapoptotic genes, such as Bax, PIG3, and PUMA, it is likely that ASPP1 and ASPP2 also stimulate the apoptotic function of p63 and p73.	transcription
58787	14	335833	5	NULL	NULL	0	NULL	ASPP1			stimulates					statement 8					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1341_s_188	14729977	Since expression of ASPP1 or ASPP2 stimulated the transactivation function of p63 and p73 on promoters of proapoptotic genes, such as Bax, PIG3, and PUMA, it is likely that ASPP1 and ASPP2 also stimulate the apoptotic function of p63 and p73.	transcription
58788	15	335833	5	NULL	NULL	0	NULL	ASPP1			stimulates					statement 9					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1341_s_188	14729977	Since expression of ASPP1 or ASPP2 stimulated the transactivation function of p63 and p73 on promoters of proapoptotic genes, such as Bax, PIG3, and PUMA, it is likely that ASPP1 and ASPP2 also stimulate the apoptotic function of p63 and p73.	transcription
58789	16	335833	5	NULL	NULL	0	NULL	ASPP2 			stimulates					statement 4					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1341_s_188	14729977	Since expression of ASPP1 or ASPP2 stimulated the transactivation function of p63 and p73 on promoters of proapoptotic genes, such as Bax, PIG3, and PUMA, it is likely that ASPP1 and ASPP2 also stimulate the apoptotic function of p63 and p73.	transcription
58790	17	335833	5	NULL	NULL	0	NULL	ASPP2			stimulates					statement 5					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1341_s_188	14729977	Since expression of ASPP1 or ASPP2 stimulated the transactivation function of p63 and p73 on promoters of proapoptotic genes, such as Bax, PIG3, and PUMA, it is likely that ASPP1 and ASPP2 also stimulate the apoptotic function of p63 and p73.	transcription
58791	18	335833	5	NULL	NULL	0	NULL	ASPP2			stimulates					statement 6					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1341_s_188	14729977	Since expression of ASPP1 or ASPP2 stimulated the transactivation function of p63 and p73 on promoters of proapoptotic genes, such as Bax, PIG3, and PUMA, it is likely that ASPP1 and ASPP2 also stimulate the apoptotic function of p63 and p73.	transcription
58792	19	335833	5	NULL	NULL	0	NULL	ASPP2			stimulates					statement 7					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1341_s_188	14729977	Since expression of ASPP1 or ASPP2 stimulated the transactivation function of p63 and p73 on promoters of proapoptotic genes, such as Bax, PIG3, and PUMA, it is likely that ASPP1 and ASPP2 also stimulate the apoptotic function of p63 and p73.	transcription
58793	20	335833	5	NULL	NULL	0	NULL	ASPP2			stimulates					statement 8					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1341_s_188	14729977	Since expression of ASPP1 or ASPP2 stimulated the transactivation function of p63 and p73 on promoters of proapoptotic genes, such as Bax, PIG3, and PUMA, it is likely that ASPP1 and ASPP2 also stimulate the apoptotic function of p63 and p73.	transcription
58794	21	335833	5	NULL	NULL	0	NULL	ASPP2			stimulates					statement 9					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1341_s_188	14729977	Since expression of ASPP1 or ASPP2 stimulated the transactivation function of p63 and p73 on promoters of proapoptotic genes, such as Bax, PIG3, and PUMA, it is likely that ASPP1 and ASPP2 also stimulate the apoptotic function of p63 and p73.	transcription
58795	22	335833	5	NULL	NULL	0	NULL	ASPP1			stimulates					p63		apoptotic function of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1341_s_188	14729977	Since expression of ASPP1 or ASPP2 stimulated the transactivation function of p63 and p73 on promoters of proapoptotic genes, such as Bax, PIG3, and PUMA, it is likely that ASPP1 and ASPP2 also stimulate the apoptotic function of p63 and p73.	transcription
58796	23	335833	5	NULL	NULL	0	NULL	ASPP2			stimulates					p63		apoptotic function of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_3_1341_s_188	14729977	Since expression of ASPP1 or ASPP2 stimulated the transactivation function of p63 and p73 on promoters of proapoptotic genes, such as Bax, PIG3, and PUMA, it is likely that ASPP1 and ASPP2 also stimulate the apoptotic function of p63 and p73.	transcription
58797	24	335833	5	NULL	NULL	0	NULL	ASPP1			stimulates					p73		apoptotic function of			NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_3_1341_s_188	14729977	Since expression of ASPP1 or ASPP2 stimulated the transactivation function of p63 and p73 on promoters of proapoptotic genes, such as Bax, PIG3, and PUMA, it is likely that ASPP1 and ASPP2 also stimulate the apoptotic function of p63 and p73.	transcription
58798	25	335833	5	NULL	NULL	0	NULL	ASPP2			stimulates					p73		apoptotic function of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1341_s_188	14729977	Since expression of ASPP1 or ASPP2 stimulated the transactivation function of p63 and p73 on promoters of proapoptotic genes, such as Bax, PIG3, and PUMA, it is likely that ASPP1 and ASPP2 also stimulate the apoptotic function of p63 and p73.	transcription
79553	1	335833	6	NULL	NULL	0	NULL	ASPP1	GP		stimulates					p63	GP	apoptotic activity of 			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1341_s_188	14729977	Since expression of ASPP1 or ASPP2 stimulated the transactivation function of p63 and p73 on promoters of proapoptotic genes, such as Bax, PIG3, and PUMA, it is likely that ASPP1 and ASPP2 also stimulate the apoptotic function of p63 and p73.	transcription
79554	2	335833	6	NULL	NULL	0	NULL	ASPP2	GP		activates					p63	GP	apoptotic activity of 			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1341_s_188	14729977	Since expression of ASPP1 or ASPP2 stimulated the transactivation function of p63 and p73 on promoters of proapoptotic genes, such as Bax, PIG3, and PUMA, it is likely that ASPP1 and ASPP2 also stimulate the apoptotic function of p63 and p73.	transcription
79555	3	335833	6	NULL	NULL	0	NULL	ASPP1	GP		stimulates					p73	GP	apoptotic activity of 			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1341_s_188	14729977	Since expression of ASPP1 or ASPP2 stimulated the transactivation function of p63 and p73 on promoters of proapoptotic genes, such as Bax, PIG3, and PUMA, it is likely that ASPP1 and ASPP2 also stimulate the apoptotic function of p63 and p73.	transcription
79556	4	335833	6	NULL	NULL	0	NULL	ASPP2	GP		stimulates					p73	GP	apoptotic activity of 			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1341_s_188	14729977	Since expression of ASPP1 or ASPP2 stimulated the transactivation function of p63 and p73 on promoters of proapoptotic genes, such as Bax, PIG3, and PUMA, it is likely that ASPP1 and ASPP2 also stimulate the apoptotic function of p63 and p73.	transcription
58799	1	335834	5	NULL	NULL	0	NULL	bax gene			is a target of		endogenous			p53					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_14_10202_s_292	10744705	WT1 Inhibits the Induction of Endogenous Mdm2 Protein by p73 and p53-- The  bax ( 48) and  mdm2 ( 57,  58) genes have been documented to be endogenous targets of p53, and p73 is also known to stimulate the expression of Mdm2 ( 45).	transcription
58800	2	335834	5	NULL	NULL	0	NULL	bax gene			is a target of		endogenous			p73					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_14_10202_s_292	10744705	WT1 Inhibits the Induction of Endogenous Mdm2 Protein by p73 and p53-- The  bax ( 48) and  mdm2 ( 57,  58) genes have been documented to be endogenous targets of p53, and p73 is also known to stimulate the expression of Mdm2 ( 45).	transcription
58801	3	335834	5	NULL	NULL	0	NULL	mdm2 gene			is a target of		endogenous			p63					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_14_10202_s_292	10744705	WT1 Inhibits the Induction of Endogenous Mdm2 Protein by p73 and p53-- The  bax ( 48) and  mdm2 ( 57,  58) genes have been documented to be endogenous targets of p53, and p73 is also known to stimulate the expression of Mdm2 ( 45).	transcription
58802	4	335834	5	NULL	NULL	0	NULL	mdm2 gene			is a target of		endogenous			p73					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_14_10202_s_292	10744705	WT1 Inhibits the Induction of Endogenous Mdm2 Protein by p73 and p53-- The  bax ( 48) and  mdm2 ( 57,  58) genes have been documented to be endogenous targets of p53, and p73 is also known to stimulate the expression of Mdm2 ( 45).	transcription
58803	5	335834	5	NULL	NULL	0	NULL	mdm2 gene			stimulates					Mdm2		expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_14_10202_s_292	10744705	WT1 Inhibits the Induction of Endogenous Mdm2 Protein by p73 and p53-- The  bax ( 48) and  mdm2 ( 57,  58) genes have been documented to be endogenous targets of p53, and p73 is also known to stimulate the expression of Mdm2 ( 45).	transcription
58804	6	335834	5	NULL	NULL	0	NULL	bax gene			stimulates					Mdm2		expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_14_10202_s_292	10744705	WT1 Inhibits the Induction of Endogenous Mdm2 Protein by p73 and p53-- The  bax ( 48) and  mdm2 ( 57,  58) genes have been documented to be endogenous targets of p53, and p73 is also known to stimulate the expression of Mdm2 ( 45).	transcription
58805	7	335834	5	NULL	NULL	0	NULL	p73			induce					Mdm2 Protein		endogenous			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_14_10202_s_292	10744705	WT1 Inhibits the Induction of Endogenous Mdm2 Protein by p73 and p53-- The  bax ( 48) and  mdm2 ( 57,  58) genes have been documented to be endogenous targets of p53, and p73 is also known to stimulate the expression of Mdm2 ( 45).	transcription
58806	8	335834	5	NULL	NULL	0	NULL	p53			induce					Mdm2 Protein		endogenous			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_14_10202_s_292	10744705	WT1 Inhibits the Induction of Endogenous Mdm2 Protein by p73 and p53-- The  bax ( 48) and  mdm2 ( 57,  58) genes have been documented to be endogenous targets of p53, and p73 is also known to stimulate the expression of Mdm2 ( 45).	transcription
58807	9	335834	5	NULL	NULL	0	NULL	WT1			inhibits					statement 7					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_14_10202_s_292	10744705	WT1 Inhibits the Induction of Endogenous Mdm2 Protein by p73 and p53-- The  bax ( 48) and  mdm2 ( 57,  58) genes have been documented to be endogenous targets of p53, and p73 is also known to stimulate the expression of Mdm2 ( 45).	transcription
58808	10	335834	5	NULL	NULL	0	NULL	WT1			inhibits					statement 8					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_14_10202_s_292	10744705	WT1 Inhibits the Induction of Endogenous Mdm2 Protein by p73 and p53-- The  bax ( 48) and  mdm2 ( 57,  58) genes have been documented to be endogenous targets of p53, and p73 is also known to stimulate the expression of Mdm2 ( 45).	transcription
79550	1	335834	6	NULL	NULL	0	NULL	p73	GP		induces					Mdm2	GP	induction of;; endogenous			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_14_10202_s_292	10744705	WT1 Inhibits the Induction of Endogenous Mdm2 Protein by p73 and p53-- The  bax ( 48) and  mdm2 ( 57,  58) genes have been documented to be endogenous targets of p53, and p73 is also known to stimulate the expression of Mdm2 ( 45).	transcription
79552	2	335834	6	NULL	NULL	0	NULL	p53	GP		induces					mdm2	GP	endogenous			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_14_10202_s_292	10744705	WT1 Inhibits the Induction of Endogenous Mdm2 Protein by p73 and p53-- The  bax ( 48) and  mdm2 ( 57,  58) genes have been documented to be endogenous targets of p53, and p73 is also known to stimulate the expression of Mdm2 ( 45).	transcription
58817	1	335835	5	NULL	NULL	0	NULL	cisplatin		transfection	upregulates					Bax		expression of			NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_11_s_193	12535517	Both cisplatin and YAP transfection-induced upregulation of Bax expression are almost completely reversed by treatment of the cells with siRNA oligonucleotides to human p73   (Figure 6A), revealing that they both require p73 function to induce the expression of the proapoptotic Bax protein in this system.	transcription
58818	2	335835	5	NULL	NULL	0	NULL	YAP		transfection	upregulates					Bax		expression of			NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_11_s_193	12535517	Both cisplatin and YAP transfection-induced upregulation of Bax expression are almost completely reversed by treatment of the cells with siRNA oligonucleotides to human p73   (Figure 6A), revealing that they both require p73 function to induce the expression of the proapoptotic Bax protein in this system.	transcription
58819	3	335835	5	NULL	NULL	0	NULL	p73 siRNA oligonucleotides		human	reverse		completely			statement 1					NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_11_s_193	12535517	Both cisplatin and YAP transfection-induced upregulation of Bax expression are almost completely reversed by treatment of the cells with siRNA oligonucleotides to human p73   (Figure 6A), revealing that they both require p73 function to induce the expression of the proapoptotic Bax protein in this system.	transcription
58820	4	335835	5	NULL	NULL	0	NULL	p73 siRNA oligonucleotides		human	reverse		completely			statement 2					NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_11_s_193	12535517	Both cisplatin and YAP transfection-induced upregulation of Bax expression are almost completely reversed by treatment of the cells with siRNA oligonucleotides to human p73   (Figure 6A), revealing that they both require p73 function to induce the expression of the proapoptotic Bax protein in this system.	transcription
58821	5	335835	5	NULL	NULL	0	NULL	statement 1			requires					p73		function of			NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_11_s_193	12535517	Both cisplatin and YAP transfection-induced upregulation of Bax expression are almost completely reversed by treatment of the cells with siRNA oligonucleotides to human p73   (Figure 6A), revealing that they both require p73 function to induce the expression of the proapoptotic Bax protein in this system.	transcription
58822	6	335835	5	NULL	NULL	0	NULL	statement 2			requires					p73		function of			NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_11_s_193	12535517	Both cisplatin and YAP transfection-induced upregulation of Bax expression are almost completely reversed by treatment of the cells with siRNA oligonucleotides to human p73   (Figure 6A), revealing that they both require p73 function to induce the expression of the proapoptotic Bax protein in this system.	transcription
58823	7	335835	5	NULL	NULL	0	NULL	Bax protein			is a type of					proapoptotic protein					NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_1_11_s_193	12535517	Both cisplatin and YAP transfection-induced upregulation of Bax expression are almost completely reversed by treatment of the cells with siRNA oligonucleotides to human p73   (Figure 6A), revealing that they both require p73 function to induce the expression of the proapoptotic Bax protein in this system.	transcription
79546	1	335835	6	NULL	NULL	0	NULL	cisplatin	Chemical		induces					Bax	GP	upregulation of			NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_11_s_193	12535517	Both cisplatin and YAP transfection-induced upregulation of Bax expression are almost completely reversed by treatment of the cells with siRNA oligonucleotides to human p73   (Figure 6A), revealing that they both require p73 function to induce the expression of the proapoptotic Bax protein in this system.	transcription
79547	2	335835	6	NULL	NULL	0	NULL	YAP	GP		induces					Bax	GP	upregulation of			NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_11_s_193	12535517	Both cisplatin and YAP transfection-induced upregulation of Bax expression are almost completely reversed by treatment of the cells with siRNA oligonucleotides to human p73   (Figure 6A), revealing that they both require p73 function to induce the expression of the proapoptotic Bax protein in this system.	transcription
79548	3	335835	6	NULL	NULL	0	NULL	p73	GP		reverses					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_11_s_193	12535517	Both cisplatin and YAP transfection-induced upregulation of Bax expression are almost completely reversed by treatment of the cells with siRNA oligonucleotides to human p73   (Figure 6A), revealing that they both require p73 function to induce the expression of the proapoptotic Bax protein in this system.	transcription
79549	4	335835	6	NULL	NULL	0	NULL	p73	GP		reverses					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_11_s_193	12535517	Both cisplatin and YAP transfection-induced upregulation of Bax expression are almost completely reversed by treatment of the cells with siRNA oligonucleotides to human p73   (Figure 6A), revealing that they both require p73 function to induce the expression of the proapoptotic Bax protein in this system.	transcription
58824	1	335836	5	NULL	NULL	0	NULL	p73			is a homolog of					p53					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_47_33747_s_246	10559267	The p53 Homolog p73 Does Not Selectively Inhibit the Ability of p53 to Activate Transcription through the bax Promoter--  In addition to BoB1 and BoB2, the p53 homolog p73 was examined as a potential explanation for the inability of wild-type p53 to activate transcription through the  bax promoter in MDA-MB-453 cells.	transcription
58825	2	335836	5	NULL	NULL	0	NULL	p53			activates					transcription					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_47_33747_s_246	10559267	The p53 Homolog p73 Does Not Selectively Inhibit the Ability of p53 to Activate Transcription through the bax Promoter--  In addition to BoB1 and BoB2, the p53 homolog p73 was examined as a potential explanation for the inability of wild-type p53 to activate transcription through the  bax promoter in MDA-MB-453 cells.	transcription
58826	3	335836	5	NULL	NULL	0	NULL	statement 2			through					bax				promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_47_33747_s_246	10559267	The p53 Homolog p73 Does Not Selectively Inhibit the Ability of p53 to Activate Transcription through the bax Promoter--  In addition to BoB1 and BoB2, the p53 homolog p73 was examined as a potential explanation for the inability of wild-type p53 to activate transcription through the  bax promoter in MDA-MB-453 cells.	transcription
58827	4	335836	5	NULL	NULL	0	NULL	p73			does not inhibit		selectively			statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_47_33747_s_246	10559267	The p53 Homolog p73 Does Not Selectively Inhibit the Ability of p53 to Activate Transcription through the bax Promoter--  In addition to BoB1 and BoB2, the p53 homolog p73 was examined as a potential explanation for the inability of wild-type p53 to activate transcription through the  bax promoter in MDA-MB-453 cells.	transcription
58828	5	335836	5	NULL	NULL	0	NULL	p53		wild-type	does not activate					transcription					NULL	MDA-MB-453 cells	0	NULL	NULL	NULL	gw60_jbiolchem_274_47_33747_s_246	10559267	The p53 Homolog p73 Does Not Selectively Inhibit the Ability of p53 to Activate Transcription through the bax Promoter--  In addition to BoB1 and BoB2, the p53 homolog p73 was examined as a potential explanation for the inability of wild-type p53 to activate transcription through the  bax promoter in MDA-MB-453 cells.	transcription
58829	6	335836	5	NULL	NULL	0	NULL	statement 5			through					bax				promoter	NULL	MDA-MB-453 cells	0	NULL	NULL	NULL	gw60_jbiolchem_274_47_33747_s_246	10559267	The p53 Homolog p73 Does Not Selectively Inhibit the Ability of p53 to Activate Transcription through the bax Promoter--  In addition to BoB1 and BoB2, the p53 homolog p73 was examined as a potential explanation for the inability of wild-type p53 to activate transcription through the  bax promoter in MDA-MB-453 cells.	transcription
58830	7	335836	5	NULL	NULL	0	NULL	p73			is responsible for					statement 5					NULL	MDA-MB-453 cells	0	NULL	NULL	NULL	gw60_jbiolchem_274_47_33747_s_246	10559267	The p53 Homolog p73 Does Not Selectively Inhibit the Ability of p53 to Activate Transcription through the bax Promoter--  In addition to BoB1 and BoB2, the p53 homolog p73 was examined as a potential explanation for the inability of wild-type p53 to activate transcription through the  bax promoter in MDA-MB-453 cells.	transcription
58831	8	335836	5	NULL	NULL	0	NULL	BoB1			is responsible for					statement 5					NULL	MDA-MB-453 cells	0	NULL	NULL	NULL	gw60_jbiolchem_274_47_33747_s_246	10559267	The p53 Homolog p73 Does Not Selectively Inhibit the Ability of p53 to Activate Transcription through the bax Promoter--  In addition to BoB1 and BoB2, the p53 homolog p73 was examined as a potential explanation for the inability of wild-type p53 to activate transcription through the  bax promoter in MDA-MB-453 cells.	transcription
58832	9	335836	5	NULL	NULL	0	NULL	BoB2			is responsible for					statement 5					NULL	MDA-MB-453 cells	0	NULL	NULL	NULL	gw60_jbiolchem_274_47_33747_s_246	10559267	The p53 Homolog p73 Does Not Selectively Inhibit the Ability of p53 to Activate Transcription through the bax Promoter--  In addition to BoB1 and BoB2, the p53 homolog p73 was examined as a potential explanation for the inability of wild-type p53 to activate transcription through the  bax promoter in MDA-MB-453 cells.	transcription
79544	1	335836	6	NULL	NULL	0	NULL	p53	GP		activates					Bax	GP			promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_47_33747_s_246	10559267	The p53 Homolog p73 Does Not Selectively Inhibit the Ability of p53 to Activate Transcription through the bax Promoter--  In addition to BoB1 and BoB2, the p53 homolog p73 was examined as a potential explanation for the inability of wild-type p53 to activate transcription through the  bax promoter in MDA-MB-453 cells.	transcription
79545	2	335836	6	NULL	NULL	0	NULL	p73	GP		does not inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_47_33747_s_246	10559267	The p53 Homolog p73 Does Not Selectively Inhibit the Ability of p53 to Activate Transcription through the bax Promoter--  In addition to BoB1 and BoB2, the p53 homolog p73 was examined as a potential explanation for the inability of wild-type p53 to activate transcription through the  bax promoter in MDA-MB-453 cells.	transcription
58833	1	335837	5	NULL	NULL	0	NULL	p73			induces					apoptosis					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_248	14634023	However, transactivation of the  bax promoter by p73gamma or p53 was observed only after 72-96 h, much later than p73- and p53-mediated induction of apoptosis.	transcription
58834	2	335837	5	NULL	NULL	0	NULL	p53			induces					apoptosis					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_248	14634023	However, transactivation of the  bax promoter by p73gamma or p53 was observed only after 72-96 h, much later than p73- and p53-mediated induction of apoptosis.	transcription
58835	3	335837	5	NULL	NULL	0	NULL	p73gamma			transactivates					bax				promoter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_248	14634023	However, transactivation of the  bax promoter by p73gamma or p53 was observed only after 72-96 h, much later than p73- and p53-mediated induction of apoptosis.	transcription
58836	4	335837	5	NULL	NULL	0	NULL	p53			transactivates					bax				promoter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_248	14634023	However, transactivation of the  bax promoter by p73gamma or p53 was observed only after 72-96 h, much later than p73- and p53-mediated induction of apoptosis.	transcription
58837	5	335837	5	NULL	NULL	0	NULL	statement 3			occurs after					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_248	14634023	However, transactivation of the  bax promoter by p73gamma or p53 was observed only after 72-96 h, much later than p73- and p53-mediated induction of apoptosis.	transcription
58838	6	335837	5	NULL	NULL	0	NULL	statement 4			occurs after					statement 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_248	14634023	However, transactivation of the  bax promoter by p73gamma or p53 was observed only after 72-96 h, much later than p73- and p53-mediated induction of apoptosis.	transcription
79542	1	335837	6	NULL	NULL	0	NULL	p73gamma	GP		transactivates					bax	GP			promoter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_248	14634023	However, transactivation of the  bax promoter by p73gamma or p53 was observed only after 72-96 h, much later than p73- and p53-mediated induction of apoptosis.	transcription
79543	2	335837	6	NULL	NULL	0	NULL	p53	GP		activates					Bax	GP			promoter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_248	14634023	However, transactivation of the  bax promoter by p73gamma or p53 was observed only after 72-96 h, much later than p73- and p53-mediated induction of apoptosis.	transcription
58839	1	335838	5	NULL	NULL	0	NULL	RDCs			activates					p53					NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_315_3_1403_s_235	16169939	We further identified several molecular mechanisms induced by RDCs, such as activation of p53 and p73, expression of p21 and Bax, induction of caspase-3, and nuclear fragmentation.	transcription
58840	2	335838	5	NULL	NULL	0	NULL	RDCs			activates					p73					NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_315_3_1403_s_235	16169939	We further identified several molecular mechanisms induced by RDCs, such as activation of p53 and p73, expression of p21 and Bax, induction of caspase-3, and nuclear fragmentation.	transcription
58841	3	335838	5	NULL	NULL	0	NULL	RDCs			induce					p21		expression of			NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_315_3_1403_s_235	16169939	We further identified several molecular mechanisms induced by RDCs, such as activation of p53 and p73, expression of p21 and Bax, induction of caspase-3, and nuclear fragmentation.	transcription
58842	4	335838	5	NULL	NULL	0	NULL	RDCs			induce					Bax		expression of			NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_315_3_1403_s_235	16169939	We further identified several molecular mechanisms induced by RDCs, such as activation of p53 and p73, expression of p21 and Bax, induction of caspase-3, and nuclear fragmentation.	transcription
58843	5	335838	5	NULL	NULL	0	NULL	RDCs			induce					caspase-3					NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_315_3_1403_s_235	16169939	We further identified several molecular mechanisms induced by RDCs, such as activation of p53 and p73, expression of p21 and Bax, induction of caspase-3, and nuclear fragmentation.	transcription
58844	6	335838	5	NULL	NULL	0	NULL	RDCs			induce					nuclear fragmentation					NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_315_3_1403_s_235	16169939	We further identified several molecular mechanisms induced by RDCs, such as activation of p53 and p73, expression of p21 and Bax, induction of caspase-3, and nuclear fragmentation.	transcription
79536	1	335838	6	NULL	NULL	0	NULL	RDC	GP		activates					p53	GP				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_315_3_1403_s_235	16169939	We further identified several molecular mechanisms induced by RDCs, such as activation of p53 and p73, expression of p21 and Bax, induction of caspase-3, and nuclear fragmentation.	transcription
79537	2	335838	6	NULL	NULL	0	NULL	RDC	GP		activates					p73	GP				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_315_3_1403_s_235	16169939	We further identified several molecular mechanisms induced by RDCs, such as activation of p53 and p73, expression of p21 and Bax, induction of caspase-3, and nuclear fragmentation.	transcription
79538	3	335838	6	NULL	NULL	0	NULL	RDC	GP		activates					p21	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_315_3_1403_s_235	16169939	We further identified several molecular mechanisms induced by RDCs, such as activation of p53 and p73, expression of p21 and Bax, induction of caspase-3, and nuclear fragmentation.	transcription
79539	4	335838	6	NULL	NULL	0	NULL	RDC	GP		activates					Bax	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_315_3_1403_s_235	16169939	We further identified several molecular mechanisms induced by RDCs, such as activation of p53 and p73, expression of p21 and Bax, induction of caspase-3, and nuclear fragmentation.	transcription
79540	5	335838	6	NULL	NULL	0	NULL	RDC	GP		activates					caspase-3	GP	induction of			NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_315_3_1403_s_235	16169939	We further identified several molecular mechanisms induced by RDCs, such as activation of p53 and p73, expression of p21 and Bax, induction of caspase-3, and nuclear fragmentation.	transcription
79541	6	335838	6	NULL	NULL	0	NULL	RDC	GP		activates					nuclear fragmentation	Process				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_315_3_1403_s_235	16169939	We further identified several molecular mechanisms induced by RDCs, such as activation of p53 and p73, expression of p21 and Bax, induction of caspase-3, and nuclear fragmentation.	transcription
58845	1	335839	5	NULL	NULL	0	NULL	CDDP			is					cisplatin					NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_11_s_199	12535517	(A) Bax protein expression induced by both cisplatin (CDDP) treatment and YAP expression is dramatically reduced by treatment with human p73 siRNA (hp73) but not control siRNA (cont).	transcription
58846	2	335839	5	NULL	NULL	0	NULL	cisplatin 		treatment	induce					Bax protein		expression of			NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_11_s_199	12535517	(A) Bax protein expression induced by both cisplatin (CDDP) treatment and YAP expression is dramatically reduced by treatment with human p73 siRNA (hp73) but not control siRNA (cont).	transcription
58847	3	335839	5	NULL	NULL	0	NULL	YAP		expression of	induce					Bax protein		expression of			NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_11_s_199	12535517	(A) Bax protein expression induced by both cisplatin (CDDP) treatment and YAP expression is dramatically reduced by treatment with human p73 siRNA (hp73) but not control siRNA (cont).	transcription
58848	4	335839	5	NULL	NULL	0	NULL	p73 siRNA		treatment;;human	reduce		dramatically			statement 2					NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_11_s_199	12535517	(A) Bax protein expression induced by both cisplatin (CDDP) treatment and YAP expression is dramatically reduced by treatment with human p73 siRNA (hp73) but not control siRNA (cont).	transcription
58849	5	335839	5	NULL	NULL	0	NULL	p73 siRNA		treatment;;human	reduce		dramatically			statement 3					NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_11_s_199	12535517	(A) Bax protein expression induced by both cisplatin (CDDP) treatment and YAP expression is dramatically reduced by treatment with human p73 siRNA (hp73) but not control siRNA (cont).	transcription
58850	6	335839	5	NULL	NULL	0	NULL	siRNA		treatment;;control	does not reduce					statement 2					NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_11_s_199	12535517	(A) Bax protein expression induced by both cisplatin (CDDP) treatment and YAP expression is dramatically reduced by treatment with human p73 siRNA (hp73) but not control siRNA (cont).	transcription
58851	7	335839	5	NULL	NULL	0	NULL	siRNA		treatment;;control	does not reduce					statement 3					NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_11_s_199	12535517	(A) Bax protein expression induced by both cisplatin (CDDP) treatment and YAP expression is dramatically reduced by treatment with human p73 siRNA (hp73) but not control siRNA (cont).	transcription
79532	1	335839	6	NULL	NULL	0	NULL	CDDP	Chemical		is					cisplatin	Chemical				NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_11_s_199	12535517	(A) Bax protein expression induced by both cisplatin (CDDP) treatment and YAP expression is dramatically reduced by treatment with human p73 siRNA (hp73) but not control siRNA (cont).	transcription
79533	2	335839	6	NULL	NULL	0	NULL	YAP	GP		increases					Bax	GP	expression of			NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_11_s_199	12535517	(A) Bax protein expression induced by both cisplatin (CDDP) treatment and YAP expression is dramatically reduced by treatment with human p73 siRNA (hp73) but not control siRNA (cont).	transcription
79534	3	335839	6	NULL	NULL	0	NULL	p73	GP		reduces					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_11_s_199	12535517	(A) Bax protein expression induced by both cisplatin (CDDP) treatment and YAP expression is dramatically reduced by treatment with human p73 siRNA (hp73) but not control siRNA (cont).	transcription
79535	4	335839	6	NULL	NULL	0	NULL	p73	GP		reduces					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_11_s_199	12535517	(A) Bax protein expression induced by both cisplatin (CDDP) treatment and YAP expression is dramatically reduced by treatment with human p73 siRNA (hp73) but not control siRNA (cont).	transcription
58852	1	335840	5	NULL	NULL	0	NULL	p53			transactivates					p21				promoter	NULL	mammalian cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_2_1438_s_255	9891077	In mammalian cells, the  GADD45 and  Bax promoters are stimulated to the same extent by all three proteins, but p53 is a more potent transactivator of  p21 and  mdm2 promoters than p73.	transcription
58853	2	335840	5	NULL	NULL	0	NULL	p53			transactivates					mdm2				promoter	NULL	mammalian cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_2_1438_s_255	9891077	In mammalian cells, the  GADD45 and  Bax promoters are stimulated to the same extent by all three proteins, but p53 is a more potent transactivator of  p21 and  mdm2 promoters than p73.	transcription
58854	3	335840	5	NULL	NULL	0	NULL	p73			transactivates					p21				promoter	NULL	mammalian cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_2_1438_s_255	9891077	In mammalian cells, the  GADD45 and  Bax promoters are stimulated to the same extent by all three proteins, but p53 is a more potent transactivator of  p21 and  mdm2 promoters than p73.	transcription
58855	4	335840	5	NULL	NULL	0	NULL	p73			transactivates					mdm2				promoter	NULL	mammalian cells	NULL	NULL	NULL	NULL	gw60_molcellbiol_19_2_1438_s_255	9891077	In mammalian cells, the  GADD45 and  Bax promoters are stimulated to the same extent by all three proteins, but p53 is a more potent transactivator of  p21 and  mdm2 promoters than p73.	transcription
58856	5	335840	5	NULL	NULL	0	NULL	statement 1			more potent than					statement 3					NULL	mammalian cells	0	NULL	NULL	NULL	gw60_molcellbiol_19_2_1438_s_255	9891077	In mammalian cells, the  GADD45 and  Bax promoters are stimulated to the same extent by all three proteins, but p53 is a more potent transactivator of  p21 and  mdm2 promoters than p73.	transcription
58857	6	335840	5	NULL	NULL	0	NULL	statement 2			more potent than					statement 4					NULL	mammalian cells	0	NULL	NULL	NULL	gw60_molcellbiol_19_2_1438_s_255	9891077	In mammalian cells, the  GADD45 and  Bax promoters are stimulated to the same extent by all three proteins, but p53 is a more potent transactivator of  p21 and  mdm2 promoters than p73.	transcription
79528	1	335840	6	NULL	NULL	0	NULL	p53	GP		transactivates					p21	GP			promoter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_2_1438_s_255	9891077	In mammalian cells, the  GADD45 and  Bax promoters are stimulated to the same extent by all three proteins, but p53 is a more potent transactivator of  p21 and  mdm2 promoters than p73.	transcription
79529	2	335840	6	NULL	NULL	0	NULL	p53	GP		transactivates					mdm2	GP			promoter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_2_1438_s_255	9891077	In mammalian cells, the  GADD45 and  Bax promoters are stimulated to the same extent by all three proteins, but p53 is a more potent transactivator of  p21 and  mdm2 promoters than p73.	transcription
79530	3	335840	6	NULL	NULL	0	NULL	p73	GP		transactivates					p21	GP			promoter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_2_1438_s_255	9891077	In mammalian cells, the  GADD45 and  Bax promoters are stimulated to the same extent by all three proteins, but p53 is a more potent transactivator of  p21 and  mdm2 promoters than p73.	transcription
79531	4	335840	6	NULL	NULL	0	NULL	p73	GP		transactivates					mdm2	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_2_1438_s_255	9891077	In mammalian cells, the  GADD45 and  Bax promoters are stimulated to the same extent by all three proteins, but p53 is a more potent transactivator of  p21 and  mdm2 promoters than p73.	transcription
58858	1	335841	5	NULL	NULL	0	NULL	p53			activates		efficiently			Bax				reporter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_259	10207112	We first compared the effects of CMV-p53 and CMV-p73 on different reporter constructs and found that both p53 and p73 could very efficiently activate the Bax and IGF-BP3 reporter constructs, while the activation of the p21Waf1 and cyclin G reporter constructs by p73 was significantly lower than that by p53.	transcription
58859	2	335841	5	NULL	NULL	0	NULL	p53			activates		efficiently			IGF-BP3				reporter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_259	10207112	We first compared the effects of CMV-p53 and CMV-p73 on different reporter constructs and found that both p53 and p73 could very efficiently activate the Bax and IGF-BP3 reporter constructs, while the activation of the p21Waf1 and cyclin G reporter constructs by p73 was significantly lower than that by p53.	transcription
58860	3	335841	5	NULL	NULL	0	NULL	p73			activates		efficiently			Bax				reporter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_259	10207112	We first compared the effects of CMV-p53 and CMV-p73 on different reporter constructs and found that both p53 and p73 could very efficiently activate the Bax and IGF-BP3 reporter constructs, while the activation of the p21Waf1 and cyclin G reporter constructs by p73 was significantly lower than that by p53.	transcription
58861	4	335841	5	NULL	NULL	0	NULL	p73			activates		efficiently			IGF-BP3				reporter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_259	10207112	We first compared the effects of CMV-p53 and CMV-p73 on different reporter constructs and found that both p53 and p73 could very efficiently activate the Bax and IGF-BP3 reporter constructs, while the activation of the p21Waf1 and cyclin G reporter constructs by p73 was significantly lower than that by p53.	transcription
58862	5	335841	5	NULL	NULL	0	NULL	p73			activates					p21Waf1				reporter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_259	10207112	We first compared the effects of CMV-p53 and CMV-p73 on different reporter constructs and found that both p53 and p73 could very efficiently activate the Bax and IGF-BP3 reporter constructs, while the activation of the p21Waf1 and cyclin G reporter constructs by p73 was significantly lower than that by p53.	transcription
58863	6	335841	5	NULL	NULL	0	NULL	p73			activates					cyclin G				reporter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_259	10207112	We first compared the effects of CMV-p53 and CMV-p73 on different reporter constructs and found that both p53 and p73 could very efficiently activate the Bax and IGF-BP3 reporter constructs, while the activation of the p21Waf1 and cyclin G reporter constructs by p73 was significantly lower than that by p53.	transcription
58864	7	335841	5	NULL	NULL	0	NULL	p53			activates					p21Waf1				reporter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_259	10207112	We first compared the effects of CMV-p53 and CMV-p73 on different reporter constructs and found that both p53 and p73 could very efficiently activate the Bax and IGF-BP3 reporter constructs, while the activation of the p21Waf1 and cyclin G reporter constructs by p73 was significantly lower than that by p53.	transcription
58865	8	335841	5	NULL	NULL	0	NULL	p53			activates					cyclin G				reporter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_259	10207112	We first compared the effects of CMV-p53 and CMV-p73 on different reporter constructs and found that both p53 and p73 could very efficiently activate the Bax and IGF-BP3 reporter constructs, while the activation of the p21Waf1 and cyclin G reporter constructs by p73 was significantly lower than that by p53.	transcription
58866	9	335841	5	NULL	NULL	0	NULL	statement 5			lower than		significantly			statement 7					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_259	10207112	We first compared the effects of CMV-p53 and CMV-p73 on different reporter constructs and found that both p53 and p73 could very efficiently activate the Bax and IGF-BP3 reporter constructs, while the activation of the p21Waf1 and cyclin G reporter constructs by p73 was significantly lower than that by p53.	transcription
58867	10	335841	5	NULL	NULL	0	NULL	statement 6			lower than		significantly			statement 8					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_259	10207112	We first compared the effects of CMV-p53 and CMV-p73 on different reporter constructs and found that both p53 and p73 could very efficiently activate the Bax and IGF-BP3 reporter constructs, while the activation of the p21Waf1 and cyclin G reporter constructs by p73 was significantly lower than that by p53.	transcription
79522	1	335841	6	NULL	NULL	0	NULL	p53	GP		activates					Bax 	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_259	10207112	We first compared the effects of CMV-p53 and CMV-p73 on different reporter constructs and found that both p53 and p73 could very efficiently activate the Bax and IGF-BP3 reporter constructs, while the activation of the p21Waf1 and cyclin G reporter constructs by p73 was significantly lower than that by p53.	transcription
79523	2	335841	6	NULL	NULL	0	NULL	p73	GP		activates					IGF-BP3	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_259	10207112	We first compared the effects of CMV-p53 and CMV-p73 on different reporter constructs and found that both p53 and p73 could very efficiently activate the Bax and IGF-BP3 reporter constructs, while the activation of the p21Waf1 and cyclin G reporter constructs by p73 was significantly lower than that by p53.	transcription
79524	3	335841	6	NULL	NULL	0	NULL	p73	GP		activates					p21Waf1	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_259	10207112	We first compared the effects of CMV-p53 and CMV-p73 on different reporter constructs and found that both p53 and p73 could very efficiently activate the Bax and IGF-BP3 reporter constructs, while the activation of the p21Waf1 and cyclin G reporter constructs by p73 was significantly lower than that by p53.	transcription
79525	4	335841	6	NULL	NULL	NULL	NULL	p73	GP		activates					cyclin G	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_259	10207112	We first compared the effects of CMV-p53 and CMV-p73 on different reporter constructs and found that both p53 and p73 could very efficiently activate the Bax and IGF-BP3 reporter constructs, while the activation of the p21Waf1 and cyclin G reporter constructs by p73 was significantly lower than that by p53.	transcription
79526	5	335841	6	NULL	NULL	0	NULL	p53	GP		activates					p21Waf1	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_259	10207112	We first compared the effects of CMV-p53 and CMV-p73 on different reporter constructs and found that both p53 and p73 could very efficiently activate the Bax and IGF-BP3 reporter constructs, while the activation of the p21Waf1 and cyclin G reporter constructs by p73 was significantly lower than that by p53.	transcription
79527	6	335841	6	NULL	NULL	0	NULL	p53	GP		activates					cyclin G	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_259	10207112	We first compared the effects of CMV-p53 and CMV-p73 on different reporter constructs and found that both p53 and p73 could very efficiently activate the Bax and IGF-BP3 reporter constructs, while the activation of the p21Waf1 and cyclin G reporter constructs by p73 was significantly lower than that by p53.	transcription
58868	1	335842	5	NULL	NULL	0	NULL	CDDP			induce					DNA		damage of			NULL		0	NULL	NULL	NULL	gw70_cellbiol_172_4_589_s_157	16461361	In this case, DNA damage induced by CDDP leads to activation of p73, and the transcription cofactor YAP promotes p73-mediated transactivation of cell death genes, including Bax and possibly PUMA ( ).	transcription
58869	2	335842	5	NULL	NULL	0	NULL	statement 1			activates					p73					NULL		0	NULL	NULL	NULL	gw70_cellbiol_172_4_589_s_157	16461361	In this case, DNA damage induced by CDDP leads to activation of p73, and the transcription cofactor YAP promotes p73-mediated transactivation of cell death genes, including Bax and possibly PUMA ( ).	transcription
58870	3	335842	5	NULL	NULL	0	NULL	p73			mediates					Bax		transactivation of			NULL		0	NULL	NULL	NULL	gw70_cellbiol_172_4_589_s_157	16461361	In this case, DNA damage induced by CDDP leads to activation of p73, and the transcription cofactor YAP promotes p73-mediated transactivation of cell death genes, including Bax and possibly PUMA ( ).	transcription
58871	4	335842	5	NULL	NULL	0	NULL	p73			mediates					PUMA		transactivation of			NULL		NULL	NULL	NULL	NULL	gw70_cellbiol_172_4_589_s_157	16461361	In this case, DNA damage induced by CDDP leads to activation of p73, and the transcription cofactor YAP promotes p73-mediated transactivation of cell death genes, including Bax and possibly PUMA ( ).	transcription
58872	5	335842	5	NULL	NULL	0	NULL	YAP			promotes					statement 3					NULL		0	NULL	NULL	NULL	gw70_cellbiol_172_4_589_s_157	16461361	In this case, DNA damage induced by CDDP leads to activation of p73, and the transcription cofactor YAP promotes p73-mediated transactivation of cell death genes, including Bax and possibly PUMA ( ).	transcription
58873	6	335842	5	NULL	NULL	0	NULL	YAP			promotes		possibly			statement 4					NULL		0	NULL	NULL	NULL	gw70_cellbiol_172_4_589_s_157	16461361	In this case, DNA damage induced by CDDP leads to activation of p73, and the transcription cofactor YAP promotes p73-mediated transactivation of cell death genes, including Bax and possibly PUMA ( ).	transcription
58874	7	335842	5	NULL	NULL	0	NULL	YAP			is a type of					transcription cofactor					NULL		0	NULL	NULL	NULL	gw70_cellbiol_172_4_589_s_157	16461361	In this case, DNA damage induced by CDDP leads to activation of p73, and the transcription cofactor YAP promotes p73-mediated transactivation of cell death genes, including Bax and possibly PUMA ( ).	transcription
58875	8	335842	5	NULL	NULL	0	NULL	Bax			is a type of					cell death gene					NULL		0	NULL	NULL	NULL	gw70_cellbiol_172_4_589_s_157	16461361	In this case, DNA damage induced by CDDP leads to activation of p73, and the transcription cofactor YAP promotes p73-mediated transactivation of cell death genes, including Bax and possibly PUMA ( ).	transcription
58876	9	335842	5	NULL	NULL	0	NULL	PUMA			is a type of					cell death gene					NULL		0	NULL	NULL	NULL	gw70_cellbiol_172_4_589_s_157	16461361	In this case, DNA damage induced by CDDP leads to activation of p73, and the transcription cofactor YAP promotes p73-mediated transactivation of cell death genes, including Bax and possibly PUMA ( ).	transcription
79517	1	335842	6	NULL	NULL	0	NULL	CDDP	GP		induces					DNA	NucleicAcid	damage to			NULL		0	NULL	NULL	NULL	gw70_cellbiol_172_4_589_s_157	16461361	In this case, DNA damage induced by CDDP leads to activation of p73, and the transcription cofactor YAP promotes p73-mediated transactivation of cell death genes, including Bax and possibly PUMA ( ).	transcription
79518	2	335842	6	NULL	NULL	0	NULL	statement 1	Process		leads to					p73	GP	activation of 			NULL		0	NULL	NULL	NULL	gw70_cellbiol_172_4_589_s_157	16461361	In this case, DNA damage induced by CDDP leads to activation of p73, and the transcription cofactor YAP promotes p73-mediated transactivation of cell death genes, including Bax and possibly PUMA ( ).	transcription
79519	3	335842	6	NULL	NULL	0	NULL	YAP	GP		is a type of					transcription cofactor	GP				NULL		0	NULL	NULL	NULL	gw70_cellbiol_172_4_589_s_157	16461361	In this case, DNA damage induced by CDDP leads to activation of p73, and the transcription cofactor YAP promotes p73-mediated transactivation of cell death genes, including Bax and possibly PUMA ( ).	transcription
79520	4	335842	6	NULL	NULL	0	NULL	p73	GP		mediates					Bax	GP	transactivation of 			NULL		0	NULL	NULL	NULL	gw70_cellbiol_172_4_589_s_157	16461361	In this case, DNA damage induced by CDDP leads to activation of p73, and the transcription cofactor YAP promotes p73-mediated transactivation of cell death genes, including Bax and possibly PUMA ( ).	transcription
79521	5	335842	6	NULL	NULL	0	NULL	YAP	GP		promotes					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_cellbiol_172_4_589_s_157	16461361	In this case, DNA damage induced by CDDP leads to activation of p73, and the transcription cofactor YAP promotes p73-mediated transactivation of cell death genes, including Bax and possibly PUMA ( ).	transcription
58877	1	335843	5	NULL	NULL	0	NULL	TNF-alpha-CHX			activates		possibly			p73		transcription function of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_10_4438_s_134	15121862	To determine if TNF-alpha-CHX activated the transcription function of p73, we performed luciferase reporter assays using promoters of either  p21CIP1 or  BAX in transient-cotransfection experiments.	transcription
58878	1	335844	5	NULL	NULL	0	NULL	YAP			stimulates					Bax		expression of			NULL	HeLa cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_25_26300_s_171	15096513	Because HeLa cells express significant amounts of p73 ( ), we tested whether co-expression of hnRNP U had an effect on the ability of YAP to stimulate the expression of Bax.	transcription
58879	2	335844	5	NULL	NULL	0	NULL	HeLa cells			express					p73					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_25_26300_s_171	15096513	Because HeLa cells express significant amounts of p73 ( ), we tested whether co-expression of hnRNP U had an effect on the ability of YAP to stimulate the expression of Bax.	transcription
58880	3	335844	5	NULL	NULL	0	NULL	hnRNP U		co-expression of	effects		possibly			statement 1					NULL	HeLa cells	0	NULL	NULL	NULL	gw70_jbiolchem_279_25_26300_s_171	15096513	Because HeLa cells express significant amounts of p73 ( ), we tested whether co-expression of hnRNP U had an effect on the ability of YAP to stimulate the expression of Bax.	transcription
79516	1	335844	6	NULL	NULL	0	NULL	YAP	GP		stimulates					Bax	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_25_26300_s_171	15096513	Because HeLa cells express significant amounts of p73 ( ), we tested whether co-expression of hnRNP U had an effect on the ability of YAP to stimulate the expression of Bax.	transcription
58881	1	335845	5	NULL	NULL	0	NULL	Bax			is translocated to					mitochondria					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_153	14634023	To identify the mediators through which p73 indirectly induces Bax mitochondrial translocation, we examined the modulation of several BH3-only proteins (data not shown) that bind to Bcl2/Xl via their BH3 domain, thereby inactivating their protective functions ( ,  ).	transcription
58882	2	335845	5	NULL	NULL	0	NULL	p73			induce		indirectly			statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_9_8076_s_153	14634023	To identify the mediators through which p73 indirectly induces Bax mitochondrial translocation, we examined the modulation of several BH3-only proteins (data not shown) that bind to Bcl2/Xl via their BH3 domain, thereby inactivating their protective functions ( ,  ).	transcription
58883	1	335846	5	NULL	NULL	0	NULL	p21/WAF-1			is a type of					p53 target gene					NULL		0	NULL	NULL	NULL	gw60_cancercell_1_4_311_s_12	12086844	Moreover, at least in overexpression assays, p63 and p73 were shown to transactivate many p53 target genes including p21/WAF-1 and Bax, and they were able to induce cell cycle arrest and apoptosis ( Yang and McKeon, 2000  ).	transcription
58884	2	335846	5	NULL	NULL	0	NULL	Bax			is a type of					p53 target gene					NULL		0	NULL	NULL	NULL	gw60_cancercell_1_4_311_s_12	12086844	Moreover, at least in overexpression assays, p63 and p73 were shown to transactivate many p53 target genes including p21/WAF-1 and Bax, and they were able to induce cell cycle arrest and apoptosis ( Yang and McKeon, 2000  ).	transcription
58885	3	335846	5	NULL	NULL	0	NULL	p63		overexpression of	transactivates					p21/WAF-1					NULL		0	NULL	NULL	NULL	gw60_cancercell_1_4_311_s_12	12086844	Moreover, at least in overexpression assays, p63 and p73 were shown to transactivate many p53 target genes including p21/WAF-1 and Bax, and they were able to induce cell cycle arrest and apoptosis ( Yang and McKeon, 2000  ).	transcription
58886	4	335846	5	NULL	NULL	0	NULL	p73		overexpression of	transactivates					p21/WAF-1					NULL		0	NULL	NULL	NULL	gw60_cancercell_1_4_311_s_12	12086844	Moreover, at least in overexpression assays, p63 and p73 were shown to transactivate many p53 target genes including p21/WAF-1 and Bax, and they were able to induce cell cycle arrest and apoptosis ( Yang and McKeon, 2000  ).	transcription
58887	5	335846	5	NULL	NULL	0	NULL	p63		overexpression of	transactivates					Bax					NULL		0	NULL	NULL	NULL	gw60_cancercell_1_4_311_s_12	12086844	Moreover, at least in overexpression assays, p63 and p73 were shown to transactivate many p53 target genes including p21/WAF-1 and Bax, and they were able to induce cell cycle arrest and apoptosis ( Yang and McKeon, 2000  ).	transcription
58888	6	335846	5	NULL	NULL	0	NULL	p73		overexpression of	transactivates					Bax					NULL		0	NULL	NULL	NULL	gw60_cancercell_1_4_311_s_12	12086844	Moreover, at least in overexpression assays, p63 and p73 were shown to transactivate many p53 target genes including p21/WAF-1 and Bax, and they were able to induce cell cycle arrest and apoptosis ( Yang and McKeon, 2000  ).	transcription
58889	7	335846	5	NULL	NULL	0	NULL	p63			induce					cell cycle arrest					NULL		0	NULL	NULL	NULL	gw60_cancercell_1_4_311_s_12	12086844	Moreover, at least in overexpression assays, p63 and p73 were shown to transactivate many p53 target genes including p21/WAF-1 and Bax, and they were able to induce cell cycle arrest and apoptosis ( Yang and McKeon, 2000  ).	transcription
58890	8	335846	5	NULL	NULL	0	NULL	p63			induce					apoptosis					NULL		0	NULL	NULL	NULL	gw60_cancercell_1_4_311_s_12	12086844	Moreover, at least in overexpression assays, p63 and p73 were shown to transactivate many p53 target genes including p21/WAF-1 and Bax, and they were able to induce cell cycle arrest and apoptosis ( Yang and McKeon, 2000  ).	transcription
58891	9	335846	5	NULL	NULL	0	NULL	p73			induce					cell cycle arrest					NULL		0	NULL	NULL	NULL	gw60_cancercell_1_4_311_s_12	12086844	Moreover, at least in overexpression assays, p63 and p73 were shown to transactivate many p53 target genes including p21/WAF-1 and Bax, and they were able to induce cell cycle arrest and apoptosis ( Yang and McKeon, 2000  ).	transcription
58892	10	335846	5	NULL	NULL	0	NULL	p73			induce					apoptosis					NULL		0	NULL	NULL	NULL	gw60_cancercell_1_4_311_s_12	12086844	Moreover, at least in overexpression assays, p63 and p73 were shown to transactivate many p53 target genes including p21/WAF-1 and Bax, and they were able to induce cell cycle arrest and apoptosis ( Yang and McKeon, 2000  ).	transcription
79512	1	335846	6	NULL	NULL	0	NULL	p63	GP		induces					cell cycle arrest	Process				NULL		0	NULL	NULL	NULL	gw60_cancercell_1_4_311_s_12	12086844	Moreover, at least in overexpression assays, p63 and p73 were shown to transactivate many p53 target genes including p21/WAF-1 and Bax, and they were able to induce cell cycle arrest and apoptosis ( Yang and McKeon, 2000  ).	transcription
79513	2	335846	6	NULL	NULL	0	NULL	p63	GP		induces					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_cancercell_1_4_311_s_12	12086844	Moreover, at least in overexpression assays, p63 and p73 were shown to transactivate many p53 target genes including p21/WAF-1 and Bax, and they were able to induce cell cycle arrest and apoptosis ( Yang and McKeon, 2000  ).	transcription
79514	3	335846	6	NULL	NULL	0	NULL	p73	GP		induces					cell cycle arrest	Process				NULL		0	NULL	NULL	NULL	gw60_cancercell_1_4_311_s_12	12086844	Moreover, at least in overexpression assays, p63 and p73 were shown to transactivate many p53 target genes including p21/WAF-1 and Bax, and they were able to induce cell cycle arrest and apoptosis ( Yang and McKeon, 2000  ).	transcription
79515	4	335846	6	NULL	NULL	0	NULL	p73	GP		induces					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_cancercell_1_4_311_s_12	12086844	Moreover, at least in overexpression assays, p63 and p73 were shown to transactivate many p53 target genes including p21/WAF-1 and Bax, and they were able to induce cell cycle arrest and apoptosis ( Yang and McKeon, 2000  ).	transcription
58893	1	335847	5	NULL	NULL	0	NULL	ik3-1		co-expression of	does not affect					Bax protein		expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2951_s_194	11706030	Protein Expression of Bax and p21 Are Not Affected by Coexpression of ik3-1 or ik3-1-deltaC-- Because p53 and p73 exert their activities by transactivating and transrepressing downstream genes, we examined expression of representative downstream gene products by immunoblotting (Fig.  6).	transcription
58894	2	335847	5	NULL	NULL	0	NULL	ik3-1-deltaC		co-expression of	does not affect					Bax protein		expression of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_4_2951_s_194	11706030	Protein Expression of Bax and p21 Are Not Affected by Coexpression of ik3-1 or ik3-1-deltaC-- Because p53 and p73 exert their activities by transactivating and transrepressing downstream genes, we examined expression of representative downstream gene products by immunoblotting (Fig.  6).	transcription
58895	3	335847	5	NULL	NULL	0	NULL	statement 1			is an alternative to					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2951_s_194	11706030	Protein Expression of Bax and p21 Are Not Affected by Coexpression of ik3-1 or ik3-1-deltaC-- Because p53 and p73 exert their activities by transactivating and transrepressing downstream genes, we examined expression of representative downstream gene products by immunoblotting (Fig.  6).	transcription
58896	4	335847	5	NULL	NULL	0	NULL	ik3-1		co-expression of	does not affect					p21 protein		expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2951_s_194	11706030	Protein Expression of Bax and p21 Are Not Affected by Coexpression of ik3-1 or ik3-1-deltaC-- Because p53 and p73 exert their activities by transactivating and transrepressing downstream genes, we examined expression of representative downstream gene products by immunoblotting (Fig.  6).	transcription
58897	5	335847	5	NULL	NULL	0	NULL	ik3-1-deltaC		co-expression of	does not affect					p21 protein		expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2951_s_194	11706030	Protein Expression of Bax and p21 Are Not Affected by Coexpression of ik3-1 or ik3-1-deltaC-- Because p53 and p73 exert their activities by transactivating and transrepressing downstream genes, we examined expression of representative downstream gene products by immunoblotting (Fig.  6).	transcription
58898	6	335847	5	NULL	NULL	0	NULL	statement 4			is an alternative to					statement 5					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_4_2951_s_194	11706030	Protein Expression of Bax and p21 Are Not Affected by Coexpression of ik3-1 or ik3-1-deltaC-- Because p53 and p73 exert their activities by transactivating and transrepressing downstream genes, we examined expression of representative downstream gene products by immunoblotting (Fig.  6).	transcription
58899	1	335848	5	NULL	NULL	0	NULL	p73		ectopically expressed	transactivates					p21				promoter	NULL	p53-deficient cell lines	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_19_15720_s_38	11279015	Furthermore, when ectopically expressed, p73 can trans-activate a variety of p53 promoters ( p21,  bax,  mdm2, and  GADD45) and induce apoptosis in p53-deficient cell lines ( 45,  48,  52,  56-59).	transcription
58900	2	335848	5	NULL	NULL	0	NULL	p73		ectopically expressed	transactivates					bax				promoter	NULL	p53-deficient cell lines	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_19_15720_s_38	11279015	Furthermore, when ectopically expressed, p73 can trans-activate a variety of p53 promoters ( p21,  bax,  mdm2, and  GADD45) and induce apoptosis in p53-deficient cell lines ( 45,  48,  52,  56-59).	transcription
58901	3	335848	5	NULL	NULL	0	NULL	p73		ectopically expressed	transactivates					mdm2				promoter	NULL	p53-deficient cell lines	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_19_15720_s_38	11279015	Furthermore, when ectopically expressed, p73 can trans-activate a variety of p53 promoters ( p21,  bax,  mdm2, and  GADD45) and induce apoptosis in p53-deficient cell lines ( 45,  48,  52,  56-59).	transcription
58902	4	335848	5	NULL	NULL	0	NULL	p73		ectopically expressed	transactivates					GADD45				promoter	NULL	p53-deficient cell lines	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_19_15720_s_38	11279015	Furthermore, when ectopically expressed, p73 can trans-activate a variety of p53 promoters ( p21,  bax,  mdm2, and  GADD45) and induce apoptosis in p53-deficient cell lines ( 45,  48,  52,  56-59).	transcription
58903	5	335848	5	NULL	NULL	0	NULL	statement 1			induce					apoptosis					NULL	p53-deficient cell lines	0	NULL	NULL	NULL	gw60_jbiolchem_276_19_15720_s_38	11279015	Furthermore, when ectopically expressed, p73 can trans-activate a variety of p53 promoters ( p21,  bax,  mdm2, and  GADD45) and induce apoptosis in p53-deficient cell lines ( 45,  48,  52,  56-59).	transcription
58904	6	335848	5	NULL	NULL	0	NULL	statement 2			induce					apoptosis					NULL	p53-deficient cell lines	0	NULL	NULL	NULL	gw60_jbiolchem_276_19_15720_s_38	11279015	Furthermore, when ectopically expressed, p73 can trans-activate a variety of p53 promoters ( p21,  bax,  mdm2, and  GADD45) and induce apoptosis in p53-deficient cell lines ( 45,  48,  52,  56-59).	transcription
58905	7	335848	5	NULL	NULL	0	NULL	statement 3			induce					apoptosis					NULL	p53-deficient cell lines	0	NULL	NULL	NULL	gw60_jbiolchem_276_19_15720_s_38	11279015	Furthermore, when ectopically expressed, p73 can trans-activate a variety of p53 promoters ( p21,  bax,  mdm2, and  GADD45) and induce apoptosis in p53-deficient cell lines ( 45,  48,  52,  56-59).	transcription
58906	8	335848	5	NULL	NULL	0	NULL	statement 4			induce					apoptosis					NULL	p53-deficient cell lines	0	NULL	NULL	NULL	gw60_jbiolchem_276_19_15720_s_38	11279015	Furthermore, when ectopically expressed, p73 can trans-activate a variety of p53 promoters ( p21,  bax,  mdm2, and  GADD45) and induce apoptosis in p53-deficient cell lines ( 45,  48,  52,  56-59).	transcription
79508	1	335848	6	NULL	NULL	0	NULL	p73	GP		transactivates					p53 	GP			promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_19_15720_s_38	11279015	Furthermore, when ectopically expressed, p73 can trans-activate a variety of p53 promoters ( p21,  bax,  mdm2, and  GADD45) and induce apoptosis in p53-deficient cell lines ( 45,  48,  52,  56-59).	transcription
79509	2	335848	6	NULL	NULL	0	NULL	p73	GP		transactivates					bax	GP			promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_19_15720_s_38	11279015	Furthermore, when ectopically expressed, p73 can trans-activate a variety of p53 promoters ( p21,  bax,  mdm2, and  GADD45) and induce apoptosis in p53-deficient cell lines ( 45,  48,  52,  56-59).	transcription
79510	3	335848	6	NULL	NULL	0	NULL	p73	GP		transactivates					mdm2	GP			promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_19_15720_s_38	11279015	Furthermore, when ectopically expressed, p73 can trans-activate a variety of p53 promoters ( p21,  bax,  mdm2, and  GADD45) and induce apoptosis in p53-deficient cell lines ( 45,  48,  52,  56-59).	transcription
79511	4	335848	6	NULL	NULL	0	NULL	p73	GP		transactivates					GADD45	GP			promoter	NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_19_15720_s_38	11279015	Furthermore, when ectopically expressed, p73 can trans-activate a variety of p53 promoters ( p21,  bax,  mdm2, and  GADD45) and induce apoptosis in p53-deficient cell lines ( 45,  48,  52,  56-59).	transcription
58907	1	335849	5	NULL	NULL	0	NULL	p53			activates					Bax				reporter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_5	10207112	Our results show that the large E1B proteins very efficiently inhibited the activity of p53 on the Bax, p21Waf1, cyclin G, and MDM2 reporter constructs but had no effect on the activation of the same reporter constructs by p73, with the exception of some inhibition of the Bax promoter by Ad12 E1B.	transcription
58908	2	335849	5	NULL	NULL	0	NULL	p53			activates					p21Waf1				reporter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_5	10207112	Our results show that the large E1B proteins very efficiently inhibited the activity of p53 on the Bax, p21Waf1, cyclin G, and MDM2 reporter constructs but had no effect on the activation of the same reporter constructs by p73, with the exception of some inhibition of the Bax promoter by Ad12 E1B.	transcription
58909	3	335849	5	NULL	NULL	0	NULL	p53			activates					cyclin G				reporter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_5	10207112	Our results show that the large E1B proteins very efficiently inhibited the activity of p53 on the Bax, p21Waf1, cyclin G, and MDM2 reporter constructs but had no effect on the activation of the same reporter constructs by p73, with the exception of some inhibition of the Bax promoter by Ad12 E1B.	transcription
58910	4	335849	5	NULL	NULL	0	NULL	p53			activates					MDM2				reporter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_5	10207112	Our results show that the large E1B proteins very efficiently inhibited the activity of p53 on the Bax, p21Waf1, cyclin G, and MDM2 reporter constructs but had no effect on the activation of the same reporter constructs by p73, with the exception of some inhibition of the Bax promoter by Ad12 E1B.	transcription
58911	5	335849	5	NULL	NULL	0	NULL	E1B proteins		large	inhibits		efficiently			statement 1					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_5	10207112	Our results show that the large E1B proteins very efficiently inhibited the activity of p53 on the Bax, p21Waf1, cyclin G, and MDM2 reporter constructs but had no effect on the activation of the same reporter constructs by p73, with the exception of some inhibition of the Bax promoter by Ad12 E1B.	transcription
58912	6	335849	5	NULL	NULL	0	NULL	E1B proteins		large	inhibits		efficiently			statement 2					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_5	10207112	Our results show that the large E1B proteins very efficiently inhibited the activity of p53 on the Bax, p21Waf1, cyclin G, and MDM2 reporter constructs but had no effect on the activation of the same reporter constructs by p73, with the exception of some inhibition of the Bax promoter by Ad12 E1B.	transcription
58913	7	335849	5	NULL	NULL	0	NULL	E1B proteins		large	inhibits		efficiently			statement 3					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_5	10207112	Our results show that the large E1B proteins very efficiently inhibited the activity of p53 on the Bax, p21Waf1, cyclin G, and MDM2 reporter constructs but had no effect on the activation of the same reporter constructs by p73, with the exception of some inhibition of the Bax promoter by Ad12 E1B.	transcription
58914	8	335849	5	NULL	NULL	0	NULL	E1B proteins		large	inhibits		efficiently			statement 4					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_5	10207112	Our results show that the large E1B proteins very efficiently inhibited the activity of p53 on the Bax, p21Waf1, cyclin G, and MDM2 reporter constructs but had no effect on the activation of the same reporter constructs by p73, with the exception of some inhibition of the Bax promoter by Ad12 E1B.	transcription
58915	9	335849	5	NULL	NULL	0	NULL	p73			activates					Bax				reporter	NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_5	10207112	Our results show that the large E1B proteins very efficiently inhibited the activity of p53 on the Bax, p21Waf1, cyclin G, and MDM2 reporter constructs but had no effect on the activation of the same reporter constructs by p73, with the exception of some inhibition of the Bax promoter by Ad12 E1B.	transcription
58916	10	335849	5	NULL	NULL	0	NULL	p73			activates					p21Waf1				reporter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_5	10207112	Our results show that the large E1B proteins very efficiently inhibited the activity of p53 on the Bax, p21Waf1, cyclin G, and MDM2 reporter constructs but had no effect on the activation of the same reporter constructs by p73, with the exception of some inhibition of the Bax promoter by Ad12 E1B.	transcription
58917	11	335849	5	NULL	NULL	0	NULL	p73			activates					cyclin G 				reporter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_5	10207112	Our results show that the large E1B proteins very efficiently inhibited the activity of p53 on the Bax, p21Waf1, cyclin G, and MDM2 reporter constructs but had no effect on the activation of the same reporter constructs by p73, with the exception of some inhibition of the Bax promoter by Ad12 E1B.	transcription
58918	12	335849	5	NULL	NULL	0	NULL	p73			activates					MDM2				reporter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_5	10207112	Our results show that the large E1B proteins very efficiently inhibited the activity of p53 on the Bax, p21Waf1, cyclin G, and MDM2 reporter constructs but had no effect on the activation of the same reporter constructs by p73, with the exception of some inhibition of the Bax promoter by Ad12 E1B.	transcription
58919	13	335849	5	NULL	NULL	0	NULL	E1B proteins \t		large	does not effect					statement 10					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_5	10207112	Our results show that the large E1B proteins very efficiently inhibited the activity of p53 on the Bax, p21Waf1, cyclin G, and MDM2 reporter constructs but had no effect on the activation of the same reporter constructs by p73, with the exception of some inhibition of the Bax promoter by Ad12 E1B.	transcription
58920	14	335849	5	NULL	NULL	0	NULL	E1B proteins \t		large	does not effect					statement 11					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_5	10207112	Our results show that the large E1B proteins very efficiently inhibited the activity of p53 on the Bax, p21Waf1, cyclin G, and MDM2 reporter constructs but had no effect on the activation of the same reporter constructs by p73, with the exception of some inhibition of the Bax promoter by Ad12 E1B.	transcription
58921	15	335849	5	NULL	NULL	0	NULL	E1B proteins \t		large	does not effect					statement 12					NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_5	10207112	Our results show that the large E1B proteins very efficiently inhibited the activity of p53 on the Bax, p21Waf1, cyclin G, and MDM2 reporter constructs but had no effect on the activation of the same reporter constructs by p73, with the exception of some inhibition of the Bax promoter by Ad12 E1B.	transcription
58922	16	335849	5	NULL	NULL	0	NULL	Ad12 E1B			inhibits					Bax				promoter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3885_s_5	10207112	Our results show that the large E1B proteins very efficiently inhibited the activity of p53 on the Bax, p21Waf1, cyclin G, and MDM2 reporter constructs but had no effect on the activation of the same reporter constructs by p73, with the exception of some inhibition of the Bax promoter by Ad12 E1B.	transcription
58923	1	335850	5	NULL	NULL	0	NULL	p21			is a type of					p53 target gene					NULL		0	NULL	NULL	NULL	gw60_pnas_95_12_6681_s_29	9618472	P73 can transcriptionally activate p53 target genes such as p21 or bax-1, and induce growth suppression or apoptosis ( 34,  35).	transcription
58924	2	335850	5	NULL	NULL	0	NULL	bax-1			is a type of					p53 target gene					NULL		0	NULL	NULL	NULL	gw60_pnas_95_12_6681_s_29	9618472	P73 can transcriptionally activate p53 target genes such as p21 or bax-1, and induce growth suppression or apoptosis ( 34,  35).	transcription
58925	3	335850	5	NULL	NULL	0	NULL	p73			activates		transcriptionaly			p21					NULL		0	NULL	NULL	NULL	gw60_pnas_95_12_6681_s_29	9618472	P73 can transcriptionally activate p53 target genes such as p21 or bax-1, and induce growth suppression or apoptosis ( 34,  35).	transcription
58926	4	335850	5	NULL	NULL	0	NULL	p73			activates		transcriptionaly			bax-1					NULL		0	NULL	NULL	NULL	gw60_pnas_95_12_6681_s_29	9618472	P73 can transcriptionally activate p53 target genes such as p21 or bax-1, and induce growth suppression or apoptosis ( 34,  35).	transcription
58927	5	335850	5	NULL	NULL	0	NULL	statement 3			induce					growth suppression					NULL		NULL	NULL	NULL	NULL	gw60_pnas_95_12_6681_s_29	9618472	P73 can transcriptionally activate p53 target genes such as p21 or bax-1, and induce growth suppression or apoptosis ( 34,  35).	transcription
58928	6	335850	5	NULL	NULL	0	NULL	statement 4			induce					growth suppression					NULL		0	NULL	NULL	NULL	gw60_pnas_95_12_6681_s_29	9618472	P73 can transcriptionally activate p53 target genes such as p21 or bax-1, and induce growth suppression or apoptosis ( 34,  35).	transcription
58929	7	335850	5	NULL	NULL	0	NULL	statement 3			induce					apoptosis					NULL		0	NULL	NULL	NULL	gw60_pnas_95_12_6681_s_29	9618472	P73 can transcriptionally activate p53 target genes such as p21 or bax-1, and induce growth suppression or apoptosis ( 34,  35).	transcription
58930	8	335850	5	NULL	NULL	0	NULL	statement 4			induce					apoptosis					NULL		0	NULL	NULL	NULL	gw60_pnas_95_12_6681_s_29	9618472	P73 can transcriptionally activate p53 target genes such as p21 or bax-1, and induce growth suppression or apoptosis ( 34,  35).	transcription
79506	1	335850	6	NULL	NULL	0	NULL	p73	GP		activates					p21	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_95_12_6681_s_29	9618472	P73 can transcriptionally activate p53 target genes such as p21 or bax-1, and induce growth suppression or apoptosis ( 34,  35).	transcription
79507	2	335850	6	NULL	NULL	0	NULL	p73	GP		activates					bax-1	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_95_12_6681_s_29	9618472	P73 can transcriptionally activate p53 target genes such as p21 or bax-1, and induce growth suppression or apoptosis ( 34,  35).	transcription
58931	1	335851	5	NULL	NULL	0	NULL	RDCs		treatment	activates		may			p73					NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_315_3_1403_s_178	16169939	To confirm whether RDCs treatment leads to p53 and p73 activation, we analyzed the expression of two p53 target genes, p21 and Bax, that can account for cell growth arrest and apoptosis (Xiong et al., 1993 ; Brady and Gil-Gomez, 1998 ).	transcription
58932	2	335851	5	NULL	NULL	0	NULL	RDCs		treatment	activates		may			p53					NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_315_3_1403_s_178	16169939	To confirm whether RDCs treatment leads to p53 and p73 activation, we analyzed the expression of two p53 target genes, p21 and Bax, that can account for cell growth arrest and apoptosis (Xiong et al., 1993 ; Brady and Gil-Gomez, 1998 ).	transcription
58933	3	335851	5	NULL	NULL	0	NULL	p21			accounts for					cell growth arrest					NULL		NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_315_3_1403_s_178	16169939	To confirm whether RDCs treatment leads to p53 and p73 activation, we analyzed the expression of two p53 target genes, p21 and Bax, that can account for cell growth arrest and apoptosis (Xiong et al., 1993 ; Brady and Gil-Gomez, 1998 ).	transcription
58934	4	335851	5	NULL	NULL	0	NULL	p21			accounts for					apoptosis					NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_315_3_1403_s_178	16169939	To confirm whether RDCs treatment leads to p53 and p73 activation, we analyzed the expression of two p53 target genes, p21 and Bax, that can account for cell growth arrest and apoptosis (Xiong et al., 1993 ; Brady and Gil-Gomez, 1998 ).	transcription
58935	5	335851	5	NULL	NULL	0	NULL	Bax			accounts for					cell growth arrest					NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_315_3_1403_s_178	16169939	To confirm whether RDCs treatment leads to p53 and p73 activation, we analyzed the expression of two p53 target genes, p21 and Bax, that can account for cell growth arrest and apoptosis (Xiong et al., 1993 ; Brady and Gil-Gomez, 1998 ).	transcription
58936	6	335851	5	NULL	NULL	0	NULL	Bax			accounts for					apoptosis					NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_315_3_1403_s_178	16169939	To confirm whether RDCs treatment leads to p53 and p73 activation, we analyzed the expression of two p53 target genes, p21 and Bax, that can account for cell growth arrest and apoptosis (Xiong et al., 1993 ; Brady and Gil-Gomez, 1998 ).	transcription
58937	7	335851	5	NULL	NULL	0	NULL	Bax			is a type of					p53 target gene					NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_315_3_1403_s_178	16169939	To confirm whether RDCs treatment leads to p53 and p73 activation, we analyzed the expression of two p53 target genes, p21 and Bax, that can account for cell growth arrest and apoptosis (Xiong et al., 1993 ; Brady and Gil-Gomez, 1998 ).	transcription
58938	8	335851	5	NULL	NULL	0	NULL	p21			is a type of					p53 target gene					NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_315_3_1403_s_178	16169939	To confirm whether RDCs treatment leads to p53 and p73 activation, we analyzed the expression of two p53 target genes, p21 and Bax, that can account for cell growth arrest and apoptosis (Xiong et al., 1993 ; Brady and Gil-Gomez, 1998 ).	transcription
58939	1	335852	5	NULL	NULL	0	NULL	U2OS cells			treated with					cisplatin					NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_11_s_191	12535517	Treatment of U2OS cells with the DNA-damaging agent cisplatin (CDDP), an activator of p73 and p53 signaling   (Gong et al., 1999  ; Ono et al., 2001  ), results in an increase in endogenous Bax protein expression as visualized by Western blot   (Figure 6A) .	transcription
58940	2	335852	5	NULL	NULL	0	NULL	statement 1			increases					Bax protein		expression of;;endogenous			NULL	U2OS cells	NULL	NULL	NULL	NULL	gw60_molcell_11_1_11_s_191	12535517	Treatment of U2OS cells with the DNA-damaging agent cisplatin (CDDP), an activator of p73 and p53 signaling   (Gong et al., 1999  ; Ono et al., 2001  ), results in an increase in endogenous Bax protein expression as visualized by Western blot   (Figure 6A) .	transcription
58941	3	335852	5	NULL	NULL	0	NULL	cisplatin			is					CDDP					NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_11_s_191	12535517	Treatment of U2OS cells with the DNA-damaging agent cisplatin (CDDP), an activator of p73 and p53 signaling   (Gong et al., 1999  ; Ono et al., 2001  ), results in an increase in endogenous Bax protein expression as visualized by Western blot   (Figure 6A) .	transcription
58942	4	335852	5	NULL	NULL	0	NULL	cisplatin			is a type of					DNA-damaging agent					NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_11_s_191	12535517	Treatment of U2OS cells with the DNA-damaging agent cisplatin (CDDP), an activator of p73 and p53 signaling   (Gong et al., 1999  ; Ono et al., 2001  ), results in an increase in endogenous Bax protein expression as visualized by Western blot   (Figure 6A) .	transcription
58943	5	335852	5	NULL	NULL	0	NULL	cisplatin			activates					p73 signaling					NULL		NULL	NULL	NULL	NULL	gw60_molcell_11_1_11_s_191	12535517	Treatment of U2OS cells with the DNA-damaging agent cisplatin (CDDP), an activator of p73 and p53 signaling   (Gong et al., 1999  ; Ono et al., 2001  ), results in an increase in endogenous Bax protein expression as visualized by Western blot   (Figure 6A) .	transcription
58944	6	335852	5	NULL	NULL	0	NULL	cisplatin			activates					p53 signaling					NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_11_s_191	12535517	Treatment of U2OS cells with the DNA-damaging agent cisplatin (CDDP), an activator of p73 and p53 signaling   (Gong et al., 1999  ; Ono et al., 2001  ), results in an increase in endogenous Bax protein expression as visualized by Western blot   (Figure 6A) .	transcription
79501	1	335852	6	NULL	NULL	0	NULL	CDDP	Chemical		is					DNA-damaging agent cisplatin	Chemical				NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_11_s_191	12535517	Treatment of U2OS cells with the DNA-damaging agent cisplatin (CDDP), an activator of p73 and p53 signaling   (Gong et al., 1999  ; Ono et al., 2001  ), results in an increase in endogenous Bax protein expression as visualized by Western blot   (Figure 6A) .	transcription
79502	2	335852	6	NULL	NULL	0	NULL	CDDP	Chemical		activates					p73 signaling	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_11_s_191	12535517	Treatment of U2OS cells with the DNA-damaging agent cisplatin (CDDP), an activator of p73 and p53 signaling   (Gong et al., 1999  ; Ono et al., 2001  ), results in an increase in endogenous Bax protein expression as visualized by Western blot   (Figure 6A) .	transcription
79503	3	335852	6	NULL	NULL	0	NULL	CDDP	Chemical		activates					p53 signaling	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_11_1_11_s_191	12535517	Treatment of U2OS cells with the DNA-damaging agent cisplatin (CDDP), an activator of p73 and p53 signaling   (Gong et al., 1999  ; Ono et al., 2001  ), results in an increase in endogenous Bax protein expression as visualized by Western blot   (Figure 6A) .	transcription
79504	4	335852	6	NULL	NULL	0	NULL	CDDP	Chemical		increases					Bax protein	GP	expression of			NULL	U2OS cells	0	NULL	NULL	NULL	gw60_molcell_11_1_11_s_191	12535517	Treatment of U2OS cells with the DNA-damaging agent cisplatin (CDDP), an activator of p73 and p53 signaling   (Gong et al., 1999  ; Ono et al., 2001  ), results in an increase in endogenous Bax protein expression as visualized by Western blot   (Figure 6A) .	transcription
58945	1	335853	5	NULL	NULL	0	NULL	p63			interacts with					p21				p53-binding sites in promoter	NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_318_2_615_s_56	15120643	Furthermore, the factor demonstrated binding specificity different from those of  p63 and p73, proteins with high homology to p53; p63 and p73 interact with p53-binding  sites in the p21 and Bax promoters with similar affinity [  37,   38,   39 and   40] whereas the BC-binding factor discriminated these two sites showing much higher  affinity for the p21Waf1 site ( Fig. 1B).	transcription
58946	2	335853	5	NULL	NULL	0	NULL	p63			interacts with					Bax				p53-binding sites in promoter	NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_318_2_615_s_56	15120643	Furthermore, the factor demonstrated binding specificity different from those of  p63 and p73, proteins with high homology to p53; p63 and p73 interact with p53-binding  sites in the p21 and Bax promoters with similar affinity [  37,   38,   39 and   40] whereas the BC-binding factor discriminated these two sites showing much higher  affinity for the p21Waf1 site ( Fig. 1B).	transcription
58947	3	335853	5	NULL	NULL	0	NULL	statement 1			similar affinity as					statement 2					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_318_2_615_s_56	15120643	Furthermore, the factor demonstrated binding specificity different from those of  p63 and p73, proteins with high homology to p53; p63 and p73 interact with p53-binding  sites in the p21 and Bax promoters with similar affinity [  37,   38,   39 and   40] whereas the BC-binding factor discriminated these two sites showing much higher  affinity for the p21Waf1 site ( Fig. 1B).	transcription
58948	4	335853	5	NULL	NULL	0	NULL	p73			interacts with					p21				p53-binding sites in promoter	NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_318_2_615_s_56	15120643	Furthermore, the factor demonstrated binding specificity different from those of  p63 and p73, proteins with high homology to p53; p63 and p73 interact with p53-binding  sites in the p21 and Bax promoters with similar affinity [  37,   38,   39 and   40] whereas the BC-binding factor discriminated these two sites showing much higher  affinity for the p21Waf1 site ( Fig. 1B).	transcription
58949	5	335853	5	NULL	NULL	0	NULL	p73			interacts with					Bax				p53-binding sites in promoter	NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_318_2_615_s_56	15120643	Furthermore, the factor demonstrated binding specificity different from those of  p63 and p73, proteins with high homology to p53; p63 and p73 interact with p53-binding  sites in the p21 and Bax promoters with similar affinity [  37,   38,   39 and   40] whereas the BC-binding factor discriminated these two sites showing much higher  affinity for the p21Waf1 site ( Fig. 1B).	transcription
58950	6	335853	5	NULL	NULL	0	NULL	statement 4			similar affinity as					statement 5					NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_318_2_615_s_56	15120643	Furthermore, the factor demonstrated binding specificity different from those of  p63 and p73, proteins with high homology to p53; p63 and p73 interact with p53-binding  sites in the p21 and Bax promoters with similar affinity [  37,   38,   39 and   40] whereas the BC-binding factor discriminated these two sites showing much higher  affinity for the p21Waf1 site ( Fig. 1B).	transcription
79499	1	335853	6	NULL	NULL	0	NULL	p63	GP		bind					p21	GP			p53-binding site of promoter	NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_318_2_615_s_56	15120643	Furthermore, the factor demonstrated binding specificity different from those of  p63 and p73, proteins with high homology to p53; p63 and p73 interact with p53-binding  sites in the p21 and Bax promoters with similar affinity [  37,   38,   39 and   40] whereas the BC-binding factor discriminated these two sites showing much higher  affinity for the p21Waf1 site ( Fig. 1B).	transcription
79500	2	335853	6	NULL	NULL	0	NULL	p73	GP		bind					Bax	GP			p53-binding site of promoter	NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_318_2_615_s_56	15120643	Furthermore, the factor demonstrated binding specificity different from those of  p63 and p73, proteins with high homology to p53; p63 and p73 interact with p53-binding  sites in the p21 and Bax promoters with similar affinity [  37,   38,   39 and   40] whereas the BC-binding factor discriminated these two sites showing much higher  affinity for the p21Waf1 site ( Fig. 1B).	transcription
58951	1	335854	5	NULL	NULL	0	NULL	p73			activates					transcription					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_17_15113_s_215	11844794	Effect of MM1 on the p73-mediated Transcriptional Activation and Growth Suppression-- To determine whether or not MM1 affects the p73- or p53-dependent transcriptional activation in cells, p53/p73-responsive  Bax,  PG13, which carries 13 copies of the consensus p53-responsive element,  p21 waf1, or  MDM2-luciferase reporter construct was co-transfected with the expression plasmid for HA-p73alpha, HA-p73beta, HA-p73alpha-(1-427), or p53 in the presence or absence of the increasing amounts of FLAG-MM1 expression plasmid into p53-deficient human osteosarcoma SAOS-2 cells.	transcription
58952	2	335854	5	NULL	NULL	0	NULL	MM1			effects		may			statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_17_15113_s_215	11844794	Effect of MM1 on the p73-mediated Transcriptional Activation and Growth Suppression-- To determine whether or not MM1 affects the p73- or p53-dependent transcriptional activation in cells, p53/p73-responsive  Bax,  PG13, which carries 13 copies of the consensus p53-responsive element,  p21 waf1, or  MDM2-luciferase reporter construct was co-transfected with the expression plasmid for HA-p73alpha, HA-p73beta, HA-p73alpha-(1-427), or p53 in the presence or absence of the increasing amounts of FLAG-MM1 expression plasmid into p53-deficient human osteosarcoma SAOS-2 cells.	transcription
58953	1	335856	5	NULL	NULL	0	NULL	Gatm			catalyzes					creatine		rate-limiting step in synthesis of			NULL		0	NULL	NULL	NULL	gw70_pnas_100_8_4622_s_3	12671064	We identified  Gatm, a gene that encodes L-arginine:glycine amidinotransferase, which catalyzes the rate-limiting step in the synthesis of creatine.	transcription
58954	2	335856	5	NULL	NULL	0	NULL	Gatm			encodes					L-arginine:glycine amidinotransferase					NULL		0	NULL	NULL	NULL	gw70_pnas_100_8_4622_s_3	12671064	We identified  Gatm, a gene that encodes L-arginine:glycine amidinotransferase, which catalyzes the rate-limiting step in the synthesis of creatine.	transcription
79497	1	335856	6	NULL	NULL	0	NULL	Gatm	GP		encodes for					L-arginine:glycine amidinotransferase	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_100_8_4622_s_3	12671064	We identified  Gatm, a gene that encodes L-arginine:glycine amidinotransferase, which catalyzes the rate-limiting step in the synthesis of creatine.	transcription
79498	2	335856	6	NULL	NULL	0	NULL	Gatm	GP		catalyzes					creatine	Chemical	synthesis of 			NULL		0	NULL	NULL	NULL	gw70_pnas_100_8_4622_s_3	12671064	We identified  Gatm, a gene that encodes L-arginine:glycine amidinotransferase, which catalyzes the rate-limiting step in the synthesis of creatine.	transcription
58955	1	335857	5	NULL	NULL	0	NULL	prednisolone			inhibit					muscle contractile proteins		proteolysis			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_13_9452_s_226	10734092	Measurements of serum creatine kinase and myoglobin, along with measurements of urinary excretion of 3-methylhistidine and glycine from these patients, suggest that prednisolone inhibits proteolysis of muscle contractile proteins ( 30).	transcription
79496	1	335857	6	NULL	NULL	0	NULL	prednisolone	Chemical		inhibits					muscle contractile proteins 	GP	proteolysis of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_13_9452_s_226	10734092	Measurements of serum creatine kinase and myoglobin, along with measurements of urinary excretion of 3-methylhistidine and glycine from these patients, suggest that prednisolone inhibits proteolysis of muscle contractile proteins ( 30).	transcription
58956	1	335862	5	NULL	NULL	0	NULL	Leydig cells		primary;;immature;;porcine	secrete					dehydroepiandrosterone					NULL		0	NULL	NULL	NULL	gw60_biolreprod_69_2_592_s_353	12700195	Biochem Biophys Acta  1994 1222:71-80 [Medline]   Mauduit C, Chauvin MA, de Peretti E, Morera AM, Benahmed M.  Effect of activin A on dehydroepiandrosterone and testosterone secretion by primary immature porcine Leydig cells.	transcription
58957	2	335862	5	NULL	NULL	0	NULL	activin A			effects		potentially			statement 1					NULL		0	NULL	NULL	NULL	gw60_biolreprod_69_2_592_s_353	12700195	Biochem Biophys Acta  1994 1222:71-80 [Medline]   Mauduit C, Chauvin MA, de Peretti E, Morera AM, Benahmed M.  Effect of activin A on dehydroepiandrosterone and testosterone secretion by primary immature porcine Leydig cells.	transcription
58958	3	335862	5	NULL	NULL	0	NULL	Leydig cells		primary;;immature;;porcine	secrete					testosterone					NULL		0	NULL	NULL	NULL	gw60_biolreprod_69_2_592_s_353	12700195	Biochem Biophys Acta  1994 1222:71-80 [Medline]   Mauduit C, Chauvin MA, de Peretti E, Morera AM, Benahmed M.  Effect of activin A on dehydroepiandrosterone and testosterone secretion by primary immature porcine Leydig cells.	transcription
58959	4	335862	5	NULL	NULL	0	NULL	activin A			effects		potentially			statement 3					NULL		0	NULL	NULL	NULL	gw60_biolreprod_69_2_592_s_353	12700195	Biochem Biophys Acta  1994 1222:71-80 [Medline]   Mauduit C, Chauvin MA, de Peretti E, Morera AM, Benahmed M.  Effect of activin A on dehydroepiandrosterone and testosterone secretion by primary immature porcine Leydig cells.	transcription
58960	1	335863	5	NULL	NULL	0	NULL	DHT			is					dihydrotestosterone					NULL		0	NULL	NULL	NULL	abs-batch0650-0679_am-j-physiol-endocrinol-metab_290_5_16368782_s_4	16368782	Dihydrotestosterone  (DHT) and testosterone (T) stimulate prostate cancer cell growth, development,  and function, whereas the effects of DHT and T in prostate stromal cells,  and of dehydroepiandrosterone (DHEA) in prostate cancer or stromal cells,  are uncertain.	transcription
58961	2	335863	5	NULL	NULL	0	NULL	T			is					testosterone					NULL		0	NULL	NULL	NULL	abs-batch0650-0679_am-j-physiol-endocrinol-metab_290_5_16368782_s_4	16368782	Dihydrotestosterone  (DHT) and testosterone (T) stimulate prostate cancer cell growth, development,  and function, whereas the effects of DHT and T in prostate stromal cells,  and of dehydroepiandrosterone (DHEA) in prostate cancer or stromal cells,  are uncertain.	transcription
58962	3	335863	5	NULL	NULL	0	NULL	testosterone			stimulates					prostate cancer cell		growth of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_am-j-physiol-endocrinol-metab_290_5_16368782_s_4	16368782	Dihydrotestosterone  (DHT) and testosterone (T) stimulate prostate cancer cell growth, development,  and function, whereas the effects of DHT and T in prostate stromal cells,  and of dehydroepiandrosterone (DHEA) in prostate cancer or stromal cells,  are uncertain.	transcription
58963	4	335863	5	NULL	NULL	0	NULL	testosterone			stimulates					prostate cancer cell		development of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_am-j-physiol-endocrinol-metab_290_5_16368782_s_4	16368782	Dihydrotestosterone  (DHT) and testosterone (T) stimulate prostate cancer cell growth, development,  and function, whereas the effects of DHT and T in prostate stromal cells,  and of dehydroepiandrosterone (DHEA) in prostate cancer or stromal cells,  are uncertain.	transcription
58964	5	335863	5	NULL	NULL	0	NULL	testosterone			stimulates					prostate cancer cell		function of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_am-j-physiol-endocrinol-metab_290_5_16368782_s_4	16368782	Dihydrotestosterone  (DHT) and testosterone (T) stimulate prostate cancer cell growth, development,  and function, whereas the effects of DHT and T in prostate stromal cells,  and of dehydroepiandrosterone (DHEA) in prostate cancer or stromal cells,  are uncertain.	transcription
58965	6	335863	5	NULL	NULL	0	NULL	dihydrotestosterone			stimulates					prostate cancer cell		growth of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_am-j-physiol-endocrinol-metab_290_5_16368782_s_4	16368782	Dihydrotestosterone  (DHT) and testosterone (T) stimulate prostate cancer cell growth, development,  and function, whereas the effects of DHT and T in prostate stromal cells,  and of dehydroepiandrosterone (DHEA) in prostate cancer or stromal cells,  are uncertain.	transcription
58966	7	335863	5	NULL	NULL	0	NULL	dihydrotestosterone			stimulates					prostate cancer cell		development of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_am-j-physiol-endocrinol-metab_290_5_16368782_s_4	16368782	Dihydrotestosterone  (DHT) and testosterone (T) stimulate prostate cancer cell growth, development,  and function, whereas the effects of DHT and T in prostate stromal cells,  and of dehydroepiandrosterone (DHEA) in prostate cancer or stromal cells,  are uncertain.	transcription
58967	8	335863	5	NULL	NULL	0	NULL	dihydrotestosterone			stimulates					prostate cancer cell		function of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_am-j-physiol-endocrinol-metab_290_5_16368782_s_4	16368782	Dihydrotestosterone  (DHT) and testosterone (T) stimulate prostate cancer cell growth, development,  and function, whereas the effects of DHT and T in prostate stromal cells,  and of dehydroepiandrosterone (DHEA) in prostate cancer or stromal cells,  are uncertain.	transcription
79492	1	335863	6	NULL	NULL	0	NULL	Dihydrotestosterone	GP		stimulate					prostate cancer cell	cell	growth of 			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_am-j-physiol-endocrinol-metab_290_5_16368782_s_4	16368782	Dihydrotestosterone  (DHT) and testosterone (T) stimulate prostate cancer cell growth, development,  and function, whereas the effects of DHT and T in prostate stromal cells,  and of dehydroepiandrosterone (DHEA) in prostate cancer or stromal cells,  are uncertain.	transcription
79493	2	335863	6	NULL	NULL	0	NULL	testosterone	GP		stimulates					prostate cancer cell	cell	growth of 			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_am-j-physiol-endocrinol-metab_290_5_16368782_s_4	16368782	Dihydrotestosterone  (DHT) and testosterone (T) stimulate prostate cancer cell growth, development,  and function, whereas the effects of DHT and T in prostate stromal cells,  and of dehydroepiandrosterone (DHEA) in prostate cancer or stromal cells,  are uncertain.	transcription
79494	3	335863	6	NULL	NULL	0	NULL	testosterone	GP		is					T	GP				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_am-j-physiol-endocrinol-metab_290_5_16368782_s_4	16368782	Dihydrotestosterone  (DHT) and testosterone (T) stimulate prostate cancer cell growth, development,  and function, whereas the effects of DHT and T in prostate stromal cells,  and of dehydroepiandrosterone (DHEA) in prostate cancer or stromal cells,  are uncertain.	transcription
79495	4	335863	6	NULL	NULL	0	NULL	DHT	GP		is					Dihydrotestosterone	GP				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_am-j-physiol-endocrinol-metab_290_5_16368782_s_4	16368782	Dihydrotestosterone  (DHT) and testosterone (T) stimulate prostate cancer cell growth, development,  and function, whereas the effects of DHT and T in prostate stromal cells,  and of dehydroepiandrosterone (DHEA) in prostate cancer or stromal cells,  are uncertain.	transcription
58968	1	335865	5	NULL	NULL	0	NULL	CRH			does not modulate					CRH-R		expression of			NULL		0	NULL	NULL	NULL	gw60_pnas_99_10_7148_s_8	12011471	CRH, dehydroepiandrosterone, and 17beta-estradiol did not modulate CRH-R expression, whereas testosterone at 10 7 M down-regulated CRH-R1 and CRH-R2 mRNA expression at 6 to 24 h, and growth hormone (GH) switched CRH-R1 mRNA expression to CRH-R2 at 24 h.	transcription
58969	2	335865	5	NULL	NULL	0	NULL	dehydroepiandrosterone			does not modulate					CRH-R		expression of			NULL		0	NULL	NULL	NULL	gw60_pnas_99_10_7148_s_8	12011471	CRH, dehydroepiandrosterone, and 17beta-estradiol did not modulate CRH-R expression, whereas testosterone at 10 7 M down-regulated CRH-R1 and CRH-R2 mRNA expression at 6 to 24 h, and growth hormone (GH) switched CRH-R1 mRNA expression to CRH-R2 at 24 h.	transcription
58970	3	335865	5	NULL	NULL	0	NULL	17beta-estradiol			does not modulate					CRH-R		expression of			NULL		0	NULL	NULL	NULL	gw60_pnas_99_10_7148_s_8	12011471	CRH, dehydroepiandrosterone, and 17beta-estradiol did not modulate CRH-R expression, whereas testosterone at 10 7 M down-regulated CRH-R1 and CRH-R2 mRNA expression at 6 to 24 h, and growth hormone (GH) switched CRH-R1 mRNA expression to CRH-R2 at 24 h.	transcription
58971	4	335865	5	NULL	NULL	0	NULL	testosterone			down-regulates					CRH-R1 mRNA		expression of			NULL		0	NULL	NULL	NULL	gw60_pnas_99_10_7148_s_8	12011471	CRH, dehydroepiandrosterone, and 17beta-estradiol did not modulate CRH-R expression, whereas testosterone at 10 7 M down-regulated CRH-R1 and CRH-R2 mRNA expression at 6 to 24 h, and growth hormone (GH) switched CRH-R1 mRNA expression to CRH-R2 at 24 h.	transcription
58972	5	335865	5	NULL	NULL	0	NULL	testosterone			down-regulates					CRH-R2 mRNA		expression of			NULL		0	NULL	NULL	NULL	gw60_pnas_99_10_7148_s_8	12011471	CRH, dehydroepiandrosterone, and 17beta-estradiol did not modulate CRH-R expression, whereas testosterone at 10 7 M down-regulated CRH-R1 and CRH-R2 mRNA expression at 6 to 24 h, and growth hormone (GH) switched CRH-R1 mRNA expression to CRH-R2 at 24 h.	transcription
58973	6	335865	5	NULL	NULL	0	NULL	CRH-R1 mRNA		expression of	switched to					CRH-R2					NULL		0	NULL	NULL	NULL	gw60_pnas_99_10_7148_s_8	12011471	CRH, dehydroepiandrosterone, and 17beta-estradiol did not modulate CRH-R expression, whereas testosterone at 10 7 M down-regulated CRH-R1 and CRH-R2 mRNA expression at 6 to 24 h, and growth hormone (GH) switched CRH-R1 mRNA expression to CRH-R2 at 24 h.	transcription
58974	7	335865	5	NULL	NULL	0	NULL	growth hormone			is required for					statement 6					NULL		0	NULL	NULL	NULL	gw60_pnas_99_10_7148_s_8	12011471	CRH, dehydroepiandrosterone, and 17beta-estradiol did not modulate CRH-R expression, whereas testosterone at 10 7 M down-regulated CRH-R1 and CRH-R2 mRNA expression at 6 to 24 h, and growth hormone (GH) switched CRH-R1 mRNA expression to CRH-R2 at 24 h.	transcription
58975	8	335865	5	NULL	NULL	0	NULL	growth hormone			is					GH					NULL		0	NULL	NULL	NULL	gw60_pnas_99_10_7148_s_8	12011471	CRH, dehydroepiandrosterone, and 17beta-estradiol did not modulate CRH-R expression, whereas testosterone at 10 7 M down-regulated CRH-R1 and CRH-R2 mRNA expression at 6 to 24 h, and growth hormone (GH) switched CRH-R1 mRNA expression to CRH-R2 at 24 h.	transcription
79487	1	335865	6	NULL	NULL	NULL	NULL	testosterone	GP		downregulates					CRH-R1 mRNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_pnas_99_10_7148_s_8	12011471	CRH, dehydroepiandrosterone, and 17beta-estradiol did not modulate CRH-R expression, whereas testosterone at 10 7 M down-regulated CRH-R1 and CRH-R2 mRNA expression at 6 to 24 h, and growth hormone (GH) switched CRH-R1 mRNA expression to CRH-R2 at 24 h.	transcription
79488	2	335865	6	NULL	NULL	0	NULL	testosterone	Chemical		downregulates					CRH-R2 mRNA	NucleicAcid	expression of			NULL		0	NULL	NULL	NULL	gw60_pnas_99_10_7148_s_8	12011471	CRH, dehydroepiandrosterone, and 17beta-estradiol did not modulate CRH-R expression, whereas testosterone at 10 7 M down-regulated CRH-R1 and CRH-R2 mRNA expression at 6 to 24 h, and growth hormone (GH) switched CRH-R1 mRNA expression to CRH-R2 at 24 h.	transcription
79489	3	335865	6	NULL	NULL	0	NULL	CRH	GP		does not modulate					CRH-R	NucleicAcid	expression of			NULL		0	NULL	NULL	NULL	gw60_pnas_99_10_7148_s_8	12011471	CRH, dehydroepiandrosterone, and 17beta-estradiol did not modulate CRH-R expression, whereas testosterone at 10 7 M down-regulated CRH-R1 and CRH-R2 mRNA expression at 6 to 24 h, and growth hormone (GH) switched CRH-R1 mRNA expression to CRH-R2 at 24 h.	transcription
79490	4	335865	6	NULL	NULL	0	NULL	dehydroepiandrosterone	Chemical		does not modulate					CRH-R	NucleicAcid	expression of			NULL		0	NULL	NULL	NULL	gw60_pnas_99_10_7148_s_8	12011471	CRH, dehydroepiandrosterone, and 17beta-estradiol did not modulate CRH-R expression, whereas testosterone at 10 7 M down-regulated CRH-R1 and CRH-R2 mRNA expression at 6 to 24 h, and growth hormone (GH) switched CRH-R1 mRNA expression to CRH-R2 at 24 h.	transcription
79491	5	335865	6	NULL	NULL	0	NULL	17beta-estradiol	Chemical		does not modulate					CRH-R	NucleicAcid	expression of			NULL		0	NULL	NULL	NULL	gw60_pnas_99_10_7148_s_8	12011471	CRH, dehydroepiandrosterone, and 17beta-estradiol did not modulate CRH-R expression, whereas testosterone at 10 7 M down-regulated CRH-R1 and CRH-R2 mRNA expression at 6 to 24 h, and growth hormone (GH) switched CRH-R1 mRNA expression to CRH-R2 at 24 h.	transcription
58976	1	335869	5	NULL	NULL	0	NULL	cyclization reactions		concerted	fabricates					four-fused-ring steroid nucleus					NULL	Drosophila	NULL	NULL	NULL	NULL	gw70_annurevnutr_25_0_499_s_247	16011476	In the case of  Drosophila this metabolic inability was recently shown to be due to the absence from the genome  of coding regions for seven enzymes in the sterol branch, including lanosterol synthase,  which catalyzes the concerted cyclization reactions required to fabricate the four-fused-ring  steroid nucleus, and 7-dehydrocholesterol reductase, which synthesizes the definitive  cholesterol molecule ( 88).	transcription
58977	2	335869	5	NULL	NULL	0	NULL	lanosterol synthase			catalyzes					statement 1					NULL	Drosophila	NULL	NULL	NULL	NULL	gw70_annurevnutr_25_0_499_s_247	16011476	In the case of  Drosophila this metabolic inability was recently shown to be due to the absence from the genome  of coding regions for seven enzymes in the sterol branch, including lanosterol synthase,  which catalyzes the concerted cyclization reactions required to fabricate the four-fused-ring  steroid nucleus, and 7-dehydrocholesterol reductase, which synthesizes the definitive  cholesterol molecule ( 88).	transcription
58978	3	335869	5	NULL	NULL	0	NULL	7-dehydrocholesterol reductase			synthesize					cholesterol molecule		definitive			NULL	Drosophila	NULL	NULL	NULL	NULL	gw70_annurevnutr_25_0_499_s_247	16011476	In the case of  Drosophila this metabolic inability was recently shown to be due to the absence from the genome  of coding regions for seven enzymes in the sterol branch, including lanosterol synthase,  which catalyzes the concerted cyclization reactions required to fabricate the four-fused-ring  steroid nucleus, and 7-dehydrocholesterol reductase, which synthesizes the definitive  cholesterol molecule ( 88).	transcription
58979	1	335870	5	NULL	NULL	0	NULL	7-ketocholesterol			is a type of					oxysterol					NULL		0	NULL	NULL	NULL	gw70_annurevcelldevbiol_22_0_129_s_396	16753029	( d) Cholesterol activates ACAT1 when an oxysterol (7-ketocholesterol) is the substrate.	transcription
58980	2	335870	5	NULL	NULL	0	NULL	cholesterol			activates					ACAT1					NULL		0	NULL	NULL	NULL	gw70_annurevcelldevbiol_22_0_129_s_396	16753029	( d) Cholesterol activates ACAT1 when an oxysterol (7-ketocholesterol) is the substrate.	transcription
58981	3	335870	5	NULL	NULL	0	NULL	7-ketocholesterol			is a substrate for					statement 2					NULL		0	NULL	NULL	NULL	gw70_annurevcelldevbiol_22_0_129_s_396	16753029	( d) Cholesterol activates ACAT1 when an oxysterol (7-ketocholesterol) is the substrate.	transcription
79485	1	335870	6	NULL	NULL	0	NULL	cholesterol	Chemical		activates					ACAT1	GP				NULL		0	NULL	NULL	NULL	gw70_annurevcelldevbiol_22_0_129_s_396	16753029	( d) Cholesterol activates ACAT1 when an oxysterol (7-ketocholesterol) is the substrate.	transcription
79486	2	335870	6	NULL	NULL	0	NULL	statement 1	Process		occurs in presence of					oxysterol	Chemical				NULL		0	NULL	NULL	NULL	gw70_annurevcelldevbiol_22_0_129_s_396	16753029	( d) Cholesterol activates ACAT1 when an oxysterol (7-ketocholesterol) is the substrate.	transcription
58982	1	335871	5	NULL	NULL	0	NULL	cholesterol efflux		macrophage foam cells	is induced by					apoA-I					NULL		0	NULL	NULL	NULL	gw60_jlipidres_40_9_1636_s_3	10484610	For example, 7-ketocholesterol (7KC) inhibits cholesterol efflux from macrophage foam cells induced by apolipoprotein A-I (apoA-I).	transcription
58983	2	335871	5	NULL	NULL	0	NULL	apoA-I			is					apolipoprotein A-I					NULL		0	NULL	NULL	NULL	gw60_jlipidres_40_9_1636_s_3	10484610	For example, 7-ketocholesterol (7KC) inhibits cholesterol efflux from macrophage foam cells induced by apolipoprotein A-I (apoA-I).	transcription
58984	3	335871	5	NULL	NULL	0	NULL	7KC			is					7-ketocholesterol					NULL		0	NULL	NULL	NULL	gw60_jlipidres_40_9_1636_s_3	10484610	For example, 7-ketocholesterol (7KC) inhibits cholesterol efflux from macrophage foam cells induced by apolipoprotein A-I (apoA-I).	transcription
58985	4	335871	5	NULL	NULL	0	NULL	7KC			inhibit					statement 1					NULL		0	NULL	NULL	NULL	gw60_jlipidres_40_9_1636_s_3	10484610	For example, 7-ketocholesterol (7KC) inhibits cholesterol efflux from macrophage foam cells induced by apolipoprotein A-I (apoA-I).	transcription
79481	1	335871	6	NULL	NULL	0	NULL	apolipoprotein A-I	GP		induces					macrophage foam cells 	Cell				NULL		0	NULL	NULL	NULL	gw60_jlipidres_40_9_1636_s_3	10484610	For example, 7-ketocholesterol (7KC) inhibits cholesterol efflux from macrophage foam cells induced by apolipoprotein A-I (apoA-I).	transcription
79482	2	335871	6	NULL	NULL	0	NULL	7-ketocholesterol	Chemical		inhibits					cholesterol	Chemical	efflux of 			NULL	macrophage foam cell	0	NULL	NULL	NULL	gw60_jlipidres_40_9_1636_s_3	10484610	For example, 7-ketocholesterol (7KC) inhibits cholesterol efflux from macrophage foam cells induced by apolipoprotein A-I (apoA-I).	transcription
79483	3	335871	6	NULL	NULL	0	NULL	7-ketocholesterol	Chemical		is					7KC	Chemical				NULL		0	NULL	NULL	NULL	gw60_jlipidres_40_9_1636_s_3	10484610	For example, 7-ketocholesterol (7KC) inhibits cholesterol efflux from macrophage foam cells induced by apolipoprotein A-I (apoA-I).	transcription
79484	4	335871	6	NULL	NULL	0	NULL	apoA-I	GP		is					apolipoprotein A-I 	GP				NULL		0	NULL	NULL	NULL	gw60_jlipidres_40_9_1636_s_3	10484610	For example, 7-ketocholesterol (7KC) inhibits cholesterol efflux from macrophage foam cells induced by apolipoprotein A-I (apoA-I).	transcription
58986	1	335872	5	NULL	NULL	0	NULL	death pathway			is mediated by					Fas					NULL		0	NULL	NULL	NULL	abs-batch0530-0539_j-mol-cell-cardiol_39_5_16198370_s_4	16198370	In  this study, we investigated whether 7-ketocholesterol, one of the major  cholesterol oxides in the lesions, altered resistance of HVSMC to Fas-mediated  death pathway.	transcription
58987	2	335872	5	NULL	NULL	0	NULL	HVSMC			resistant to					statement 1					NULL		0	NULL	NULL	NULL	abs-batch0530-0539_j-mol-cell-cardiol_39_5_16198370_s_4	16198370	In  this study, we investigated whether 7-ketocholesterol, one of the major  cholesterol oxides in the lesions, altered resistance of HVSMC to Fas-mediated  death pathway.	transcription
58988	3	335872	5	NULL	NULL	0	NULL	7-ketocholesterol			alter		may			statement 2					NULL		0	NULL	NULL	NULL	abs-batch0530-0539_j-mol-cell-cardiol_39_5_16198370_s_4	16198370	In  this study, we investigated whether 7-ketocholesterol, one of the major  cholesterol oxides in the lesions, altered resistance of HVSMC to Fas-mediated  death pathway.	transcription
58989	4	335872	5	NULL	NULL	0	NULL	7-ketocholesterol			is a type of					cholesterol oxides					NULL	lesions	0	NULL	NULL	NULL	abs-batch0530-0539_j-mol-cell-cardiol_39_5_16198370_s_4	16198370	In  this study, we investigated whether 7-ketocholesterol, one of the major  cholesterol oxides in the lesions, altered resistance of HVSMC to Fas-mediated  death pathway.	transcription
79480	1	335872	6	NULL	NULL	0	NULL	HVSMC	Cell		is resistant to					Fas-mediated death pathway	Process				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_j-mol-cell-cardiol_39_5_16198370_s_4	16198370	In  this study, we investigated whether 7-ketocholesterol, one of the major  cholesterol oxides in the lesions, altered resistance of HVSMC to Fas-mediated  death pathway.	transcription
58990	1	335873	5	NULL	NULL	0	NULL	oxysterols			effects		may			SMC DNA		synthesis of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_194_s_150	8620332	Effect of Oxysterols on SMC DNA Synthesis    xidation of LDL is associated with increased accumulation of a number of oxysterols, such as 5alpha,6alpha-epoxy cholesterol, cholestane-3beta,5alpha,6beta-triol, 7alpha-hydroxycholesterol, 7beta-hydroxycholesterol, 7-ketocholesterol, 24-hydroxycholesterol, 25-hydroxycholesterol, and 27-hydroxycholesterol.	transcription
58991	2	335873	5	NULL	NULL	0	NULL	LDL		oxidation of	is associated with					5alpha,6alpha-epoxy cholesterol		increased accumulation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_194_s_150	8620332	Effect of Oxysterols on SMC DNA Synthesis    xidation of LDL is associated with increased accumulation of a number of oxysterols, such as 5alpha,6alpha-epoxy cholesterol, cholestane-3beta,5alpha,6beta-triol, 7alpha-hydroxycholesterol, 7beta-hydroxycholesterol, 7-ketocholesterol, 24-hydroxycholesterol, 25-hydroxycholesterol, and 27-hydroxycholesterol.	transcription
58992	3	335873	5	NULL	NULL	0	NULL	LDL		oxidation of	is associated with					cholestane-3beta,5alpha,6beta-triol		increased accumulation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_194_s_150	8620332	Effect of Oxysterols on SMC DNA Synthesis    xidation of LDL is associated with increased accumulation of a number of oxysterols, such as 5alpha,6alpha-epoxy cholesterol, cholestane-3beta,5alpha,6beta-triol, 7alpha-hydroxycholesterol, 7beta-hydroxycholesterol, 7-ketocholesterol, 24-hydroxycholesterol, 25-hydroxycholesterol, and 27-hydroxycholesterol.	transcription
58993	4	335873	5	NULL	NULL	0	NULL	LDL		oxidation of	is associated with					7alpha-hydroxycholesterol		increased accumulation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_194_s_150	8620332	Effect of Oxysterols on SMC DNA Synthesis    xidation of LDL is associated with increased accumulation of a number of oxysterols, such as 5alpha,6alpha-epoxy cholesterol, cholestane-3beta,5alpha,6beta-triol, 7alpha-hydroxycholesterol, 7beta-hydroxycholesterol, 7-ketocholesterol, 24-hydroxycholesterol, 25-hydroxycholesterol, and 27-hydroxycholesterol.	transcription
58994	5	335873	5	NULL	NULL	0	NULL	LDL		oxidation of	is associated with					7beta-hydroxycholesterol		increased accumulation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_194_s_150	8620332	Effect of Oxysterols on SMC DNA Synthesis    xidation of LDL is associated with increased accumulation of a number of oxysterols, such as 5alpha,6alpha-epoxy cholesterol, cholestane-3beta,5alpha,6beta-triol, 7alpha-hydroxycholesterol, 7beta-hydroxycholesterol, 7-ketocholesterol, 24-hydroxycholesterol, 25-hydroxycholesterol, and 27-hydroxycholesterol.	transcription
58995	6	335873	5	NULL	NULL	0	NULL	LDL		oxidation of	is associated with					7-ketocholesterol		increased accumulation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_194_s_150	8620332	Effect of Oxysterols on SMC DNA Synthesis    xidation of LDL is associated with increased accumulation of a number of oxysterols, such as 5alpha,6alpha-epoxy cholesterol, cholestane-3beta,5alpha,6beta-triol, 7alpha-hydroxycholesterol, 7beta-hydroxycholesterol, 7-ketocholesterol, 24-hydroxycholesterol, 25-hydroxycholesterol, and 27-hydroxycholesterol.	transcription
58996	7	335873	5	NULL	NULL	0	NULL	LDL		oxidation of	is associated with					24-hydroxycholesterol		increased accumulation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_194_s_150	8620332	Effect of Oxysterols on SMC DNA Synthesis    xidation of LDL is associated with increased accumulation of a number of oxysterols, such as 5alpha,6alpha-epoxy cholesterol, cholestane-3beta,5alpha,6beta-triol, 7alpha-hydroxycholesterol, 7beta-hydroxycholesterol, 7-ketocholesterol, 24-hydroxycholesterol, 25-hydroxycholesterol, and 27-hydroxycholesterol.	transcription
58997	8	335873	5	NULL	NULL	0	NULL	LDL		oxidation of	is associated with					25-hydroxycholesterol		increased accumulation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_194_s_150	8620332	Effect of Oxysterols on SMC DNA Synthesis    xidation of LDL is associated with increased accumulation of a number of oxysterols, such as 5alpha,6alpha-epoxy cholesterol, cholestane-3beta,5alpha,6beta-triol, 7alpha-hydroxycholesterol, 7beta-hydroxycholesterol, 7-ketocholesterol, 24-hydroxycholesterol, 25-hydroxycholesterol, and 27-hydroxycholesterol.	transcription
58998	9	335873	5	NULL	NULL	0	NULL	LDL		oxidation of	is associated with					27-hydroxycholesterol		increased accumulation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_194_s_150	8620332	Effect of Oxysterols on SMC DNA Synthesis    xidation of LDL is associated with increased accumulation of a number of oxysterols, such as 5alpha,6alpha-epoxy cholesterol, cholestane-3beta,5alpha,6beta-triol, 7alpha-hydroxycholesterol, 7beta-hydroxycholesterol, 7-ketocholesterol, 24-hydroxycholesterol, 25-hydroxycholesterol, and 27-hydroxycholesterol.	transcription
58999	10	335873	5	NULL	NULL	0	NULL	5alpha,6alpha-epoxy cholesterol			is a type of					oxysterol					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_194_s_150	8620332	Effect of Oxysterols on SMC DNA Synthesis    xidation of LDL is associated with increased accumulation of a number of oxysterols, such as 5alpha,6alpha-epoxy cholesterol, cholestane-3beta,5alpha,6beta-triol, 7alpha-hydroxycholesterol, 7beta-hydroxycholesterol, 7-ketocholesterol, 24-hydroxycholesterol, 25-hydroxycholesterol, and 27-hydroxycholesterol.	transcription
59000	11	335873	5	NULL	NULL	0	NULL	cholestane-3beta,5alpha,6beta-triol			is a type of					oxysterol					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_194_s_150	8620332	Effect of Oxysterols on SMC DNA Synthesis    xidation of LDL is associated with increased accumulation of a number of oxysterols, such as 5alpha,6alpha-epoxy cholesterol, cholestane-3beta,5alpha,6beta-triol, 7alpha-hydroxycholesterol, 7beta-hydroxycholesterol, 7-ketocholesterol, 24-hydroxycholesterol, 25-hydroxycholesterol, and 27-hydroxycholesterol.	transcription
59001	12	335873	5	NULL	NULL	0	NULL	7alpha-hydroxycholesterol			is a type of					oxysterol					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_194_s_150	8620332	Effect of Oxysterols on SMC DNA Synthesis    xidation of LDL is associated with increased accumulation of a number of oxysterols, such as 5alpha,6alpha-epoxy cholesterol, cholestane-3beta,5alpha,6beta-triol, 7alpha-hydroxycholesterol, 7beta-hydroxycholesterol, 7-ketocholesterol, 24-hydroxycholesterol, 25-hydroxycholesterol, and 27-hydroxycholesterol.	transcription
59002	13	335873	5	NULL	NULL	0	NULL	7beta-hydroxycholesterol			is a type of					oxysterol					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_194_s_150	8620332	Effect of Oxysterols on SMC DNA Synthesis    xidation of LDL is associated with increased accumulation of a number of oxysterols, such as 5alpha,6alpha-epoxy cholesterol, cholestane-3beta,5alpha,6beta-triol, 7alpha-hydroxycholesterol, 7beta-hydroxycholesterol, 7-ketocholesterol, 24-hydroxycholesterol, 25-hydroxycholesterol, and 27-hydroxycholesterol.	transcription
59003	14	335873	5	NULL	NULL	0	NULL	7-ketocholesterol			is a type of					oxysterol					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_194_s_150	8620332	Effect of Oxysterols on SMC DNA Synthesis    xidation of LDL is associated with increased accumulation of a number of oxysterols, such as 5alpha,6alpha-epoxy cholesterol, cholestane-3beta,5alpha,6beta-triol, 7alpha-hydroxycholesterol, 7beta-hydroxycholesterol, 7-ketocholesterol, 24-hydroxycholesterol, 25-hydroxycholesterol, and 27-hydroxycholesterol.	transcription
59004	15	335873	5	NULL	NULL	0	NULL	24-hydroxycholesterol			is a type of					oxysterol					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_194_s_150	8620332	Effect of Oxysterols on SMC DNA Synthesis    xidation of LDL is associated with increased accumulation of a number of oxysterols, such as 5alpha,6alpha-epoxy cholesterol, cholestane-3beta,5alpha,6beta-triol, 7alpha-hydroxycholesterol, 7beta-hydroxycholesterol, 7-ketocholesterol, 24-hydroxycholesterol, 25-hydroxycholesterol, and 27-hydroxycholesterol.	transcription
59005	16	335873	5	NULL	NULL	0	NULL	25-hydroxycholesterol			is a type of					oxysterol					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_194_s_150	8620332	Effect of Oxysterols on SMC DNA Synthesis    xidation of LDL is associated with increased accumulation of a number of oxysterols, such as 5alpha,6alpha-epoxy cholesterol, cholestane-3beta,5alpha,6beta-triol, 7alpha-hydroxycholesterol, 7beta-hydroxycholesterol, 7-ketocholesterol, 24-hydroxycholesterol, 25-hydroxycholesterol, and 27-hydroxycholesterol.	transcription
59006	17	335873	5	NULL	NULL	0	NULL	27-hydroxycholesterol			is a type of					oxysterol					NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_194_s_150	8620332	Effect of Oxysterols on SMC DNA Synthesis    xidation of LDL is associated with increased accumulation of a number of oxysterols, such as 5alpha,6alpha-epoxy cholesterol, cholestane-3beta,5alpha,6beta-triol, 7alpha-hydroxycholesterol, 7beta-hydroxycholesterol, 7-ketocholesterol, 24-hydroxycholesterol, 25-hydroxycholesterol, and 27-hydroxycholesterol.	transcription
79479	1	335873	6	NULL	NULL	0	NULL	LDL	Chemical	oxidation of 	is associated with					oxysterol	Chemical	accumulation of 			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_16_2_194_s_150	8620332	Effect of Oxysterols on SMC DNA Synthesis    xidation of LDL is associated with increased accumulation of a number of oxysterols, such as 5alpha,6alpha-epoxy cholesterol, cholestane-3beta,5alpha,6beta-triol, 7alpha-hydroxycholesterol, 7beta-hydroxycholesterol, 7-ketocholesterol, 24-hydroxycholesterol, 25-hydroxycholesterol, and 27-hydroxycholesterol.	transcription
59007	1	335874	5	NULL	NULL	0	NULL	ACAT			is					acyl-CoA:cholesterol acyltransferase					NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_9_1844_s_144	9741697	To determine whether the acyl-CoA:cholesterol acyltransferase (ACAT) activity was inhibited by CPHS, we tested the effect of this steroid in the presence of 7-ketocholesterol which is known to be an ACAT substrate  ( 16).	transcription
59008	2	335874	5	NULL	NULL	0	NULL	ACAT		activity of	is inhibited by		may be			CPHS					NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_9_1844_s_144	9741697	To determine whether the acyl-CoA:cholesterol acyltransferase (ACAT) activity was inhibited by CPHS, we tested the effect of this steroid in the presence of 7-ketocholesterol which is known to be an ACAT substrate  ( 16).	transcription
59009	3	335874	5	NULL	NULL	0	NULL	7-ketocholesterol			is a substrate of					ACAT 					NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_9_1844_s_144	9741697	To determine whether the acyl-CoA:cholesterol acyltransferase (ACAT) activity was inhibited by CPHS, we tested the effect of this steroid in the presence of 7-ketocholesterol which is known to be an ACAT substrate  ( 16).	transcription
59010	1	335876	5	NULL	NULL	0	NULL	sphingosine			activates					PLD					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_25_15579_s_93	9188441	In contrast to ceramides, sphingosine and its metabolite sphingosine-1-P activate PLD ( 58).	transcription
59011	2	335876	5	NULL	NULL	0	NULL	sphingosine-1-P			activates					PLD					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_25_15579_s_93	9188441	In contrast to ceramides, sphingosine and its metabolite sphingosine-1-P activate PLD ( 58).	transcription
59012	3	335876	5	NULL	NULL	0	NULL	sphingosine-1-P			is a metabolite of					sphingosine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_25_15579_s_93	9188441	In contrast to ceramides, sphingosine and its metabolite sphingosine-1-P activate PLD ( 58).	transcription
59013	4	335876	5	NULL	NULL	0	NULL	ceramides			does not activate					PLD					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_25_15579_s_93	9188441	In contrast to ceramides, sphingosine and its metabolite sphingosine-1-P activate PLD ( 58).	transcription
59014	1	335877	5	NULL	NULL	0	NULL	sphingosine			induce					ceramide		accumulation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_165	15774472	Sphingosine induces ceramide accumulation.	transcription
79478	1	335877	6	NULL	NULL	0	NULL	sphingosine	Chemical		induces					Ceramide	Chemical	accumulation of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_165	15774472	Sphingosine induces ceramide accumulation.	transcription
59015	1	335878	5	NULL	NULL	0	NULL	SPP			is degraded to					sphingosine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_297	7592842	Ceramides  stimulate the degradation of SPP to sphingosine and ceramide and  stimulate the production of ceramides from endogenous lipids.	transcription
59016	2	335878	5	NULL	NULL	0	NULL	SPP			is degraded to					ceramide					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_297	7592842	Ceramides  stimulate the degradation of SPP to sphingosine and ceramide and  stimulate the production of ceramides from endogenous lipids.	transcription
59017	3	335878	5	NULL	NULL	0	NULL	statement 1			occurs simultaneously with					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_297	7592842	Ceramides  stimulate the degradation of SPP to sphingosine and ceramide and  stimulate the production of ceramides from endogenous lipids.	transcription
59018	4	335878	5	NULL	NULL	0	NULL	ceramides			stimulates					statement 3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_297	7592842	Ceramides  stimulate the degradation of SPP to sphingosine and ceramide and  stimulate the production of ceramides from endogenous lipids.	transcription
59019	5	335878	5	NULL	NULL	0	NULL	ceramides			is produced from					lipids		endogenous			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_297	7592842	Ceramides  stimulate the degradation of SPP to sphingosine and ceramide and  stimulate the production of ceramides from endogenous lipids.	transcription
59020	6	335878	5	NULL	NULL	0	NULL	ceramides			stimulates					statement 5					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_297	7592842	Ceramides  stimulate the degradation of SPP to sphingosine and ceramide and  stimulate the production of ceramides from endogenous lipids.	transcription
79473	1	335878	6	NULL	NULL	0	NULL	SPP	GP		degrades into					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_297	7592842	Ceramides  stimulate the degradation of SPP to sphingosine and ceramide and  stimulate the production of ceramides from endogenous lipids.	transcription
79474	2	335878	6	NULL	NULL	0	NULL	SPP	GP		degrades into					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_297	7592842	Ceramides  stimulate the degradation of SPP to sphingosine and ceramide and  stimulate the production of ceramides from endogenous lipids.	transcription
79475	3	335878	6	NULL	NULL	0	NULL	Ceramides	Chemical		stimulates					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_297	7592842	Ceramides  stimulate the degradation of SPP to sphingosine and ceramide and  stimulate the production of ceramides from endogenous lipids.	transcription
79476	4	335878	6	NULL	NULL	0	NULL	Ceramides	Chemical		stimulates					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_297	7592842	Ceramides  stimulate the degradation of SPP to sphingosine and ceramide and  stimulate the production of ceramides from endogenous lipids.	transcription
79477	5	335878	6	NULL	NULL	0	NULL	lipids	Chemical	endogenous	produces					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_297	7592842	Ceramides  stimulate the degradation of SPP to sphingosine and ceramide and  stimulate the production of ceramides from endogenous lipids.	transcription
59021	1	335879	5	NULL	NULL	0	NULL	palmitate			stimulates					ceramide		accumulation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_80	15774472	Palmitate stimulates ceramide and sphingosine accumulation.	transcription
59022	2	335879	5	NULL	NULL	0	NULL	palmitate			stimulates					sphingosine		accumulation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_80	15774472	Palmitate stimulates ceramide and sphingosine accumulation.	transcription
79471	1	335879	6	NULL	NULL	0	NULL	Palmitate	Chemical		stimulates					ceramide	Chemical	accumulation of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_80	15774472	Palmitate stimulates ceramide and sphingosine accumulation.	transcription
79472	2	335879	6	NULL	NULL	0	NULL	palmitate	Chemical		stimulates					sphingosine	Chemical	accumulation of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_80	15774472	Palmitate stimulates ceramide and sphingosine accumulation.	transcription
59023	1	335880	5	NULL	NULL	0	NULL	PLD			is stimulated by					sphingosine 1-phosphate					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_200	7592842	Figure 5:Effect of okadaic acid on the stimulation  of PLD by sphingosine 1-phosphate and the production of endogenous  ceramides by C -ceramide.	transcription
59024	2	335880	5	NULL	NULL	0	NULL	okadaic acid			effects		potentially			statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_200	7592842	Figure 5:Effect of okadaic acid on the stimulation  of PLD by sphingosine 1-phosphate and the production of endogenous  ceramides by C -ceramide.	transcription
59025	3	335880	5	NULL	NULL	0	NULL	ceramides		endogenous	is produced by					C -ceramide					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_200	7592842	Figure 5:Effect of okadaic acid on the stimulation  of PLD by sphingosine 1-phosphate and the production of endogenous  ceramides by C -ceramide.	transcription
59026	4	335880	5	NULL	NULL	0	NULL	okadaic acid			effects		potentially			statement 3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_200	7592842	Figure 5:Effect of okadaic acid on the stimulation  of PLD by sphingosine 1-phosphate and the production of endogenous  ceramides by C -ceramide.	transcription
79469	1	335880	6	NULL	NULL	0	NULL	sphingosine 1-phosphate	GP		stimulates					PLD	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_200	7592842	Figure 5:Effect of okadaic acid on the stimulation  of PLD by sphingosine 1-phosphate and the production of endogenous  ceramides by C -ceramide.	transcription
79470	2	335880	6	NULL	NULL	0	NULL	C-ceramide	Chemical		produces					ceramides	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_200	7592842	Figure 5:Effect of okadaic acid on the stimulation  of PLD by sphingosine 1-phosphate and the production of endogenous  ceramides by C -ceramide.	transcription
59027	1	335881	5	NULL	NULL	0	NULL	sphingosine			induce					apoptosis					NULL		0	NULL	NULL	NULL	gw60_febslett_425_1_61_s_46	9541007	Sphingosine and ceramide induce apoptosis without interconversion of the lipids	transcription
59028	2	335881	5	NULL	NULL	0	NULL	statement 1			without interconversion of					lipids					NULL		0	NULL	NULL	NULL	gw60_febslett_425_1_61_s_46	9541007	Sphingosine and ceramide induce apoptosis without interconversion of the lipids	transcription
59029	3	335881	5	NULL	NULL	0	NULL	ceramide			induce					apoptosis					NULL		0	NULL	NULL	NULL	gw60_febslett_425_1_61_s_46	9541007	Sphingosine and ceramide induce apoptosis without interconversion of the lipids	transcription
59030	4	335881	5	NULL	NULL	0	NULL	statement 3			without interconversion of					lipids					NULL		0	NULL	NULL	NULL	gw60_febslett_425_1_61_s_46	9541007	Sphingosine and ceramide induce apoptosis without interconversion of the lipids	transcription
79467	1	335881	6	NULL	NULL	0	NULL	sphingosine	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_425_1_61_s_46	9541007	Sphingosine and ceramide induce apoptosis without interconversion of the lipids	transcription
79468	2	335881	6	NULL	NULL	0	NULL	ceramide	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_425_1_61_s_46	9541007	Sphingosine and ceramide induce apoptosis without interconversion of the lipids	transcription
59031	1	335882	5	NULL	NULL	0	NULL	sphingosine			induce					apoptosis					NULL	WEHI 231	0	NULL	NULL	NULL	gw60_molpharmacol_61_1_177_s_346	11752219	Sphingosine and ceramide induce apoptosis in WEHI 231.	transcription
59032	2	335882	5	NULL	NULL	0	NULL	ceramide			induce					apoptosis					NULL	WEHI 231	0	NULL	NULL	NULL	gw60_molpharmacol_61_1_177_s_346	11752219	Sphingosine and ceramide induce apoptosis in WEHI 231.	transcription
79465	1	335882	6	NULL	NULL	NULL	NULL	sphingosine	Chemical		induces					apoptosis	Process				NULL	WEHI 231	NULL	NULL	NULL	NULL	gw60_molpharmacol_61_1_177_s_346	11752219	Sphingosine and ceramide induce apoptosis in WEHI 231.	transcription
79466	2	335882	6	NULL	NULL	NULL	NULL	ceramide	Chemical		induces					apoptosis	Process				NULL	WEHI 231	NULL	NULL	NULL	NULL	gw60_molpharmacol_61_1_177_s_346	11752219	Sphingosine and ceramide induce apoptosis in WEHI 231.	transcription
59033	1	335883	5	NULL	NULL	0	NULL	apoptosis			is induced by					ceramide					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_199	8626522	Figure 7: Potentiation of ceramide-induced apoptosis  by sphingosine.	transcription
59034	2	335883	5	NULL	NULL	0	NULL	sphingosine			potentiate					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_199	8626522	Figure 7: Potentiation of ceramide-induced apoptosis  by sphingosine.	transcription
79463	1	335883	6	NULL	NULL	0	NULL	ceramide	Chemical		induces					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_199	8626522	Figure 7: Potentiation of ceramide-induced apoptosis  by sphingosine.	transcription
79464	2	335883	6	NULL	NULL	0	NULL	sphingosine	Chemical		potentiates					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_199	8626522	Figure 7: Potentiation of ceramide-induced apoptosis  by sphingosine.	transcription
59035	1	335884	5	NULL	NULL	0	NULL	dSREBP		cleavage of	is inhibited by					palmitate					NULL		0	NULL	NULL	NULL	gw60_science_296_5569_879_s_76	11988566	( A) Cleavage of dSREBP is inhibited by palmitate, ceramide, or sphingosine.	transcription
59036	2	335884	5	NULL	NULL	0	NULL	dSREBP		cleavage of	is inhibited by					ceramide					NULL		0	NULL	NULL	NULL	gw60_science_296_5569_879_s_76	11988566	( A) Cleavage of dSREBP is inhibited by palmitate, ceramide, or sphingosine.	transcription
59037	3	335884	5	NULL	NULL	0	NULL	dSREBP		cleavage of	is inhibited by					sphingosine					NULL		0	NULL	NULL	NULL	gw60_science_296_5569_879_s_76	11988566	( A) Cleavage of dSREBP is inhibited by palmitate, ceramide, or sphingosine.	transcription
79460	1	335884	6	NULL	NULL	0	NULL	palmitate	Chemical		inhibits					dSREBP	GP	cleavage of 			NULL		0	NULL	NULL	NULL	gw60_science_296_5569_879_s_76	11988566	( A) Cleavage of dSREBP is inhibited by palmitate, ceramide, or sphingosine.	transcription
79461	2	335884	6	NULL	NULL	0	NULL	ceramide	Chemical		inhibits					dSREBP	GP	cleavage of 			NULL		0	NULL	NULL	NULL	gw60_science_296_5569_879_s_76	11988566	( A) Cleavage of dSREBP is inhibited by palmitate, ceramide, or sphingosine.	transcription
79462	3	335884	6	NULL	NULL	0	NULL	sphingosine	Chemical		inhibits					dSREBP	GP	cleavage of 			NULL		0	NULL	NULL	NULL	gw60_science_296_5569_879_s_76	11988566	( A) Cleavage of dSREBP is inhibited by palmitate, ceramide, or sphingosine.	transcription
59038	1	335885	5	NULL	NULL	0	NULL	ceramide			is converted to					sphingosine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_34_30784_s_7	12072440	Inhibition of ceramide conversion to sphingosine had no effect on this ceramide-induced effect.	transcription
79459	1	335885	6	NULL	NULL	0	NULL	ceramide	Chemical		is converted to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_34_30784_s_7	12072440	Inhibition of ceramide conversion to sphingosine had no effect on this ceramide-induced effect.	transcription
59039	1	335886	5	NULL	NULL	0	NULL	sphingosine		increase in	results from		may			ceramide		degradation of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_42	12531549	The ceramide increase preceded that of sphingosine, suggesting that the increase in sphingosine could result from degradation of the ceramide.	transcription
59080	1	335887	5	NULL	NULL	0	NULL	SM			is hydrolyzed by					SMase					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_340	14702348	It has been reported that the catabolic generation of ceramide is mediated by the hydrolysis of SM by SMase, that ceramide is deamidated to sphingosine by ceramidase, and that sphingosine is phosphorylated to S1P by sphingosine kinase ( ).	transcription
59081	2	335887	5	NULL	NULL	0	NULL	statement 1			generates		catabolically			ceramide					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_340	14702348	It has been reported that the catabolic generation of ceramide is mediated by the hydrolysis of SM by SMase, that ceramide is deamidated to sphingosine by ceramidase, and that sphingosine is phosphorylated to S1P by sphingosine kinase ( ).	transcription
59082	3	335887	5	NULL	NULL	0	NULL	ceramide			deamidated to					sphingosine					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_340	14702348	It has been reported that the catabolic generation of ceramide is mediated by the hydrolysis of SM by SMase, that ceramide is deamidated to sphingosine by ceramidase, and that sphingosine is phosphorylated to S1P by sphingosine kinase ( ).	transcription
59083	4	335887	5	NULL	NULL	0	NULL	ceramidase			catalyzes					statement 3					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_340	14702348	It has been reported that the catabolic generation of ceramide is mediated by the hydrolysis of SM by SMase, that ceramide is deamidated to sphingosine by ceramidase, and that sphingosine is phosphorylated to S1P by sphingosine kinase ( ).	transcription
59084	5	335887	5	NULL	NULL	0	NULL	sphingosine			is phosphorylated to					S1P					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_340	14702348	It has been reported that the catabolic generation of ceramide is mediated by the hydrolysis of SM by SMase, that ceramide is deamidated to sphingosine by ceramidase, and that sphingosine is phosphorylated to S1P by sphingosine kinase ( ).	transcription
59085	6	335887	5	NULL	NULL	0	NULL	sphingosine kinase			catalyzes					statement 5					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_340	14702348	It has been reported that the catabolic generation of ceramide is mediated by the hydrolysis of SM by SMase, that ceramide is deamidated to sphingosine by ceramidase, and that sphingosine is phosphorylated to S1P by sphingosine kinase ( ).	transcription
79453	1	335887	6	NULL	NULL	0	NULL	SM	Chemical		is hydrolysed to					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_340	14702348	It has been reported that the catabolic generation of ceramide is mediated by the hydrolysis of SM by SMase, that ceramide is deamidated to sphingosine by ceramidase, and that sphingosine is phosphorylated to S1P by sphingosine kinase ( ).	transcription
79454	2	335887	6	NULL	NULL	0	NULL	SMase	GP		catalyzes					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_340	14702348	It has been reported that the catabolic generation of ceramide is mediated by the hydrolysis of SM by SMase, that ceramide is deamidated to sphingosine by ceramidase, and that sphingosine is phosphorylated to S1P by sphingosine kinase ( ).	transcription
79455	3	335887	6	NULL	NULL	0	NULL	ceramide	Chemical		is deaminated to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_340	14702348	It has been reported that the catabolic generation of ceramide is mediated by the hydrolysis of SM by SMase, that ceramide is deamidated to sphingosine by ceramidase, and that sphingosine is phosphorylated to S1P by sphingosine kinase ( ).	transcription
79456	4	335887	6	NULL	NULL	0	NULL	ceramidase	GP		catalyzes					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_340	14702348	It has been reported that the catabolic generation of ceramide is mediated by the hydrolysis of SM by SMase, that ceramide is deamidated to sphingosine by ceramidase, and that sphingosine is phosphorylated to S1P by sphingosine kinase ( ).	transcription
79457	5	335887	6	NULL	NULL	0	NULL	sphingosine	Chemical		phosphorylates to					S1P	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_340	14702348	It has been reported that the catabolic generation of ceramide is mediated by the hydrolysis of SM by SMase, that ceramide is deamidated to sphingosine by ceramidase, and that sphingosine is phosphorylated to S1P by sphingosine kinase ( ).	transcription
79458	6	335887	6	NULL	NULL	0	NULL	statement 5	Process		occurs by					sphingosine kinase	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_340	14702348	It has been reported that the catabolic generation of ceramide is mediated by the hydrolysis of SM by SMase, that ceramide is deamidated to sphingosine by ceramidase, and that sphingosine is phosphorylated to S1P by sphingosine kinase ( ).	transcription
59086	1	335888	5	NULL	NULL	0	NULL	ceramide synthase			is a type of					ceramidase					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_46	12531549	Together with ceramide synthase and glucosylceramide synthase, ceramidases, by catalyzing the hydrolysis of ceramide to sphingosine, regulate the available supply of ceramide.	transcription
59087	2	335888	5	NULL	NULL	0	NULL	glucosylceramide synthase			is a type of					ceramidase					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_46	12531549	Together with ceramide synthase and glucosylceramide synthase, ceramidases, by catalyzing the hydrolysis of ceramide to sphingosine, regulate the available supply of ceramide.	transcription
59088	3	335888	5	NULL	NULL	0	NULL	ceramide			is hydrolyzed to					sphingosine					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_46	12531549	Together with ceramide synthase and glucosylceramide synthase, ceramidases, by catalyzing the hydrolysis of ceramide to sphingosine, regulate the available supply of ceramide.	transcription
59089	4	335888	5	NULL	NULL	0	NULL	ceramide synthase			catalyzes					statement 3					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_46	12531549	Together with ceramide synthase and glucosylceramide synthase, ceramidases, by catalyzing the hydrolysis of ceramide to sphingosine, regulate the available supply of ceramide.	transcription
59090	5	335888	5	NULL	NULL	0	NULL	glucosylceramide synthase \t			catalyzes					statement 3					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_46	12531549	Together with ceramide synthase and glucosylceramide synthase, ceramidases, by catalyzing the hydrolysis of ceramide to sphingosine, regulate the available supply of ceramide.	transcription
59091	6	335888	5	NULL	NULL	0	NULL	statement 4			regulates					ceramide		available supply of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_46	12531549	Together with ceramide synthase and glucosylceramide synthase, ceramidases, by catalyzing the hydrolysis of ceramide to sphingosine, regulate the available supply of ceramide.	transcription
59092	7	335888	5	NULL	NULL	0	NULL	statement 5			regulates					ceramide		available supply of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_46	12531549	Together with ceramide synthase and glucosylceramide synthase, ceramidases, by catalyzing the hydrolysis of ceramide to sphingosine, regulate the available supply of ceramide.	transcription
79450	1	335888	6	NULL	NULL	0	NULL	ceramide	Chemical		is converted to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_46	12531549	Together with ceramide synthase and glucosylceramide synthase, ceramidases, by catalyzing the hydrolysis of ceramide to sphingosine, regulate the available supply of ceramide.	transcription
79451	2	335888	6	NULL	NULL	0	NULL	ceramide synthase 	GP		catalyzes					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_46	12531549	Together with ceramide synthase and glucosylceramide synthase, ceramidases, by catalyzing the hydrolysis of ceramide to sphingosine, regulate the available supply of ceramide.	transcription
79452	3	335888	6	NULL	NULL	0	NULL	glucosylceramide synthase	GP		catalyzes					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_46	12531549	Together with ceramide synthase and glucosylceramide synthase, ceramidases, by catalyzing the hydrolysis of ceramide to sphingosine, regulate the available supply of ceramide.	transcription
59093	1	335889	5	NULL	NULL	0	NULL	ceramide			is a type of					sphingolipid metabolite					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_247	10747891	Ceramide and sphingosine are interconvertable sphingolipid metabolites; however, we have shown that sphingosine induces apoptosis without being converted to ceramide inasmuch as the ceramide synthase inhibitor fumonisin B1 did not affect sphingosine- or Fas-induced apoptosis.	transcription
59094	2	335889	5	NULL	NULL	0	NULL	sphingosine			is a type of					sphingolipid metabolite					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_247	10747891	Ceramide and sphingosine are interconvertable sphingolipid metabolites; however, we have shown that sphingosine induces apoptosis without being converted to ceramide inasmuch as the ceramide synthase inhibitor fumonisin B1 did not affect sphingosine- or Fas-induced apoptosis.	transcription
59095	3	335889	5	NULL	NULL	0	NULL	sphingosine			induce					apoptosis					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_247	10747891	Ceramide and sphingosine are interconvertable sphingolipid metabolites; however, we have shown that sphingosine induces apoptosis without being converted to ceramide inasmuch as the ceramide synthase inhibitor fumonisin B1 did not affect sphingosine- or Fas-induced apoptosis.	transcription
59096	4	335889	5	NULL	NULL	0	NULL	sphingosine			is not converted to					ceramide					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_247	10747891	Ceramide and sphingosine are interconvertable sphingolipid metabolites; however, we have shown that sphingosine induces apoptosis without being converted to ceramide inasmuch as the ceramide synthase inhibitor fumonisin B1 did not affect sphingosine- or Fas-induced apoptosis.	transcription
59097	5	335889	5	NULL	NULL	0	NULL	statement 4			is necessary for					statement 3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_247	10747891	Ceramide and sphingosine are interconvertable sphingolipid metabolites; however, we have shown that sphingosine induces apoptosis without being converted to ceramide inasmuch as the ceramide synthase inhibitor fumonisin B1 did not affect sphingosine- or Fas-induced apoptosis.	transcription
59115	6	335889	5	NULL	NULL	0	NULL	fumonisin B1			is an inhibitor of					ceramide synthase 					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_247	10747891	Ceramide and sphingosine are interconvertable sphingolipid metabolites; however, we have shown that sphingosine induces apoptosis without being converted to ceramide inasmuch as the ceramide synthase inhibitor fumonisin B1 did not affect sphingosine- or Fas-induced apoptosis.	transcription
59121	7	335889	5	NULL	NULL	0	NULL	apoptosis			is induced by					sphingosine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_247	10747891	Ceramide and sphingosine are interconvertable sphingolipid metabolites; however, we have shown that sphingosine induces apoptosis without being converted to ceramide inasmuch as the ceramide synthase inhibitor fumonisin B1 did not affect sphingosine- or Fas-induced apoptosis.	transcription
59122	8	335889	5	NULL	NULL	0	NULL	fumonisin B1			does not affect					statement 7					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_247	10747891	Ceramide and sphingosine are interconvertable sphingolipid metabolites; however, we have shown that sphingosine induces apoptosis without being converted to ceramide inasmuch as the ceramide synthase inhibitor fumonisin B1 did not affect sphingosine- or Fas-induced apoptosis.	transcription
59123	9	335889	5	NULL	NULL	0	NULL	apoptosis			is induced by					Fas					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_247	10747891	Ceramide and sphingosine are interconvertable sphingolipid metabolites; however, we have shown that sphingosine induces apoptosis without being converted to ceramide inasmuch as the ceramide synthase inhibitor fumonisin B1 did not affect sphingosine- or Fas-induced apoptosis.	transcription
59125	10	335889	5	NULL	NULL	0	NULL	fumonisin B1			does not affect					statement 9					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_247	10747891	Ceramide and sphingosine are interconvertable sphingolipid metabolites; however, we have shown that sphingosine induces apoptosis without being converted to ceramide inasmuch as the ceramide synthase inhibitor fumonisin B1 did not affect sphingosine- or Fas-induced apoptosis.	transcription
59126	1	335890	5	NULL	NULL	0	NULL	PAI-1 gene			is induced by					ceramide					NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_192	16936207	Genes such as PAI-1 and KC were induced by ceramide, sphingosine, and S1P.	transcription
59127	2	335890	5	NULL	NULL	0	NULL	PAI-1 gene			is induced by					sphingosine					NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_192	16936207	Genes such as PAI-1 and KC were induced by ceramide, sphingosine, and S1P.	transcription
59128	3	335890	5	NULL	NULL	0	NULL	PAI-1 gene			is induced by					S1P					NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_192	16936207	Genes such as PAI-1 and KC were induced by ceramide, sphingosine, and S1P.	transcription
59130	4	335890	5	NULL	NULL	0	NULL	KC gene			is induced by					ceramide					NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_192	16936207	Genes such as PAI-1 and KC were induced by ceramide, sphingosine, and S1P.	transcription
59131	5	335890	5	NULL	NULL	0	NULL	KC gene			is induced by					sphingosine					NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_192	16936207	Genes such as PAI-1 and KC were induced by ceramide, sphingosine, and S1P.	transcription
59132	6	335890	5	NULL	NULL	0	NULL	KC gene			is induced by					S1P					NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_192	16936207	Genes such as PAI-1 and KC were induced by ceramide, sphingosine, and S1P.	transcription
79444	1	335890	6	NULL	NULL	0	NULL	ceramide	Chemical		induces					PAI-1	GP				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_192	16936207	Genes such as PAI-1 and KC were induced by ceramide, sphingosine, and S1P.	transcription
79445	2	335890	6	NULL	NULL	0	NULL	ceramide	Chemical		induces					KC	GP				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_192	16936207	Genes such as PAI-1 and KC were induced by ceramide, sphingosine, and S1P.	transcription
79446	3	335890	6	NULL	NULL	0	NULL	sphingosine	Chemical		induces					PAI-1	GP				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_192	16936207	Genes such as PAI-1 and KC were induced by ceramide, sphingosine, and S1P.	transcription
79447	4	335890	6	NULL	NULL	0	NULL	sphingosine	Chemical		induces					KC	GP				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_192	16936207	Genes such as PAI-1 and KC were induced by ceramide, sphingosine, and S1P.	transcription
79448	5	335890	6	NULL	NULL	0	NULL	S1P	GP		induces					PAI-1	GP				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_192	16936207	Genes such as PAI-1 and KC were induced by ceramide, sphingosine, and S1P.	transcription
79449	6	335890	6	NULL	NULL	0	NULL	S1P	GP		induces					KC	GP				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_192	16936207	Genes such as PAI-1 and KC were induced by ceramide, sphingosine, and S1P.	transcription
59133	1	335891	5	NULL	NULL	0	NULL	ceramide			is hydrolyzed to					sphingosine					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_35_32978_s_16	12815059	1.23 [EC]) catalyzes the hydrolysis of  ceramide to sphingosine and fatty acid.	transcription
59135	2	335891	5	NULL	NULL	0	NULL	ceramide			is hydrolyzed to					fatty acid					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_35_32978_s_16	12815059	1.23 [EC]) catalyzes the hydrolysis of  ceramide to sphingosine and fatty acid.	transcription
59136	3	335891	5	NULL	NULL	0	NULL	statement 1			occurs along with					statement 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_35_32978_s_16	12815059	1.23 [EC]) catalyzes the hydrolysis of  ceramide to sphingosine and fatty acid.	transcription
79442	1	335891	6	NULL	NULL	0	NULL	ceramide	Chemical		is hydrolysed to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_35_32978_s_16	12815059	1.23 [EC]) catalyzes the hydrolysis of  ceramide to sphingosine and fatty acid.	transcription
79443	2	335891	6	NULL	NULL	0	NULL	ceramide	Chemical		is hydrolysed to					fatty acid 	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_35_32978_s_16	12815059	1.23 [EC]) catalyzes the hydrolysis of  ceramide to sphingosine and fatty acid.	transcription
59137	1	335892	5	NULL	NULL	0	NULL	L-Cycloserine			blocks					sphingosine		biosynthesis of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_184	12424251	L-Cycloserine blocks sphingosine and ceramide biosynthesis by inhibiting serine palmitoyltransferase activity.	transcription
59139	2	335892	5	NULL	NULL	0	NULL	L-Cycloserine			blocks					ceramide		biosynthesis of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_184	12424251	L-Cycloserine blocks sphingosine and ceramide biosynthesis by inhibiting serine palmitoyltransferase activity.	transcription
59140	3	335892	5	NULL	NULL	0	NULL	L-Cycloserine			inhibit					serine palmitoyltransferase		activity of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_184	12424251	L-Cycloserine blocks sphingosine and ceramide biosynthesis by inhibiting serine palmitoyltransferase activity.	transcription
59141	4	335892	5	NULL	NULL	0	NULL	L-Cycloserine			inhibit					serine palmitoyltransferase		activity of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_184	12424251	L-Cycloserine blocks sphingosine and ceramide biosynthesis by inhibiting serine palmitoyltransferase activity.	transcription
59142	5	335892	5	NULL	NULL	0	NULL	statement 3			leads to					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_184	12424251	L-Cycloserine blocks sphingosine and ceramide biosynthesis by inhibiting serine palmitoyltransferase activity.	transcription
59144	6	335892	5	NULL	NULL	0	NULL	statement 5			leads to					statement 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_184	12424251	L-Cycloserine blocks sphingosine and ceramide biosynthesis by inhibiting serine palmitoyltransferase activity.	transcription
79440	1	335892	6	NULL	NULL	0	NULL	L-Cycloserine	Chemical		blocks					sphingosine	Chemical	biosynthesis of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_184	12424251	L-Cycloserine blocks sphingosine and ceramide biosynthesis by inhibiting serine palmitoyltransferase activity.	transcription
79441	2	335892	6	NULL	NULL	0	NULL	L-Cycloserine	Chemical		blocks					ceramide	Chemical	biosynthesis of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_184	12424251	L-Cycloserine blocks sphingosine and ceramide biosynthesis by inhibiting serine palmitoyltransferase activity.	transcription
59147	1	335893	5	NULL	NULL	0	NULL	sphingosine			activates					PLD					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_2_291_s_128	10425402	Ceramide was shown to inhibit sphingosine and sphingosine-1-phosphate activation of PLD but not of cyclic AMP generation.	transcription
59148	2	335893	5	NULL	NULL	0	NULL	sphingosine-1-phosphate			activates					PLD					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_2_291_s_128	10425402	Ceramide was shown to inhibit sphingosine and sphingosine-1-phosphate activation of PLD but not of cyclic AMP generation.	transcription
59149	3	335893	5	NULL	NULL	0	NULL	ceramide			inhibit					statement 1					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_2_291_s_128	10425402	Ceramide was shown to inhibit sphingosine and sphingosine-1-phosphate activation of PLD but not of cyclic AMP generation.	transcription
59150	4	335893	5	NULL	NULL	0	NULL	ceramide			inhibit					statement 2					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_2_291_s_128	10425402	Ceramide was shown to inhibit sphingosine and sphingosine-1-phosphate activation of PLD but not of cyclic AMP generation.	transcription
59151	5	335893	5	NULL	NULL	0	NULL	sphingosine			activates					cyclic AMP		generation of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_2_291_s_128	10425402	Ceramide was shown to inhibit sphingosine and sphingosine-1-phosphate activation of PLD but not of cyclic AMP generation.	transcription
59152	6	335893	5	NULL	NULL	0	NULL	sphingosine-1-phosphate			activates					cyclic AMP		generation of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_2_291_s_128	10425402	Ceramide was shown to inhibit sphingosine and sphingosine-1-phosphate activation of PLD but not of cyclic AMP generation.	transcription
59153	7	335893	5	NULL	NULL	0	NULL	ceramide			inhibit					statement 5					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_2_291_s_128	10425402	Ceramide was shown to inhibit sphingosine and sphingosine-1-phosphate activation of PLD but not of cyclic AMP generation.	transcription
59154	8	335893	5	NULL	NULL	0	NULL	ceramide			inhibit					statement 6					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_2_291_s_128	10425402	Ceramide was shown to inhibit sphingosine and sphingosine-1-phosphate activation of PLD but not of cyclic AMP generation.	transcription
79438	1	335893	6	NULL	NULL	0	NULL	ceramide	Chemical		inhibits					sphingosine	Chemical	activation of 			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_2_291_s_128	10425402	Ceramide was shown to inhibit sphingosine and sphingosine-1-phosphate activation of PLD but not of cyclic AMP generation.	transcription
79439	2	335893	6	NULL	NULL	0	NULL	ceramide	Chemical		inhibits					sphingosine 1-phosphate	GP	activation of 			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_2_291_s_128	10425402	Ceramide was shown to inhibit sphingosine and sphingosine-1-phosphate activation of PLD but not of cyclic AMP generation.	transcription
59155	1	335894	5	NULL	NULL	0	NULL	ceramide			is cleaved into					sphingosine		nonradiolabeled			NULL		0	NULL	NULL	NULL	gw60_clindiagnlabimmun_6_1_101_s_68	9874672	CDase catalyzed the cleavage of [14]ceramide to nonradiolabeled sphingosine and 14C-radiolabeled palmitic acid.	transcription
59156	2	335894	5	NULL	NULL	0	NULL	ceramide			is cleaved into					palmitic acid		14C-radiolabeled			NULL		0	NULL	NULL	NULL	gw60_clindiagnlabimmun_6_1_101_s_68	9874672	CDase catalyzed the cleavage of [14]ceramide to nonradiolabeled sphingosine and 14C-radiolabeled palmitic acid.	transcription
59157	3	335894	5	NULL	NULL	0	NULL	statement 1			occurs along with					statement 2					NULL		0	NULL	NULL	NULL	gw60_clindiagnlabimmun_6_1_101_s_68	9874672	CDase catalyzed the cleavage of [14]ceramide to nonradiolabeled sphingosine and 14C-radiolabeled palmitic acid.	transcription
59158	4	335894	5	NULL	NULL	0	NULL	CDase			catalyzes					statement 3					NULL		0	NULL	NULL	NULL	gw60_clindiagnlabimmun_6_1_101_s_68	9874672	CDase catalyzed the cleavage of [14]ceramide to nonradiolabeled sphingosine and 14C-radiolabeled palmitic acid.	transcription
79436	1	335894	6	NULL	NULL	0	NULL	ceramide	Chemical		is converted to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_clindiagnlabimmun_6_1_101_s_68	9874672	CDase catalyzed the cleavage of [14]ceramide to nonradiolabeled sphingosine and 14C-radiolabeled palmitic acid.	transcription
79437	2	335894	6	NULL	NULL	0	NULL	CDase	Chemical		catalyzes					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_clindiagnlabimmun_6_1_101_s_68	9874672	CDase catalyzed the cleavage of [14]ceramide to nonradiolabeled sphingosine and 14C-radiolabeled palmitic acid.	transcription
59159	1	335895	5	NULL	NULL	0	NULL	ceramide		elevation of;;endogenous	induce					apoptosis					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_1_177_s_13	10617602	In particular, apoptosis is known to be induced by elevation of endogenous ceramide or sphingosine ( 1-10).	transcription
59160	2	335895	5	NULL	NULL	0	NULL	sphingosine		elevation of;;endogenous	induce					apoptosis					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_1_177_s_13	10617602	In particular, apoptosis is known to be induced by elevation of endogenous ceramide or sphingosine ( 1-10).	transcription
59161	3	335895	5	NULL	NULL	0	NULL	statement 1			is an alternative to					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_1_177_s_13	10617602	In particular, apoptosis is known to be induced by elevation of endogenous ceramide or sphingosine ( 1-10).	transcription
79434	1	335895	6	NULL	NULL	0	NULL	ceramide	Chemical	elevation of	induces					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_1_177_s_13	10617602	In particular, apoptosis is known to be induced by elevation of endogenous ceramide or sphingosine ( 1-10).	transcription
79435	2	335895	6	NULL	NULL	0	NULL	sphingosine	Chemical	elevation of	induces					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_1_177_s_13	10617602	In particular, apoptosis is known to be induced by elevation of endogenous ceramide or sphingosine ( 1-10).	transcription
59162	1	335896	5	NULL	NULL	0	NULL	sphingosine 1-phosphate			stimulates					PLD					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_179	7592842	Figure 4:Effect of C -ceramide on the  stimulation of PLD by sphingosine 1-phosphate.	transcription
59163	2	335896	5	NULL	NULL	0	NULL	C -ceramide			effects		may			statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_179	7592842	Figure 4:Effect of C -ceramide on the  stimulation of PLD by sphingosine 1-phosphate.	transcription
79433	1	335896	6	NULL	NULL	0	NULL	sphingosine 1-phosphate	GP		stimulates					PLD	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_179	7592842	Figure 4:Effect of C -ceramide on the  stimulation of PLD by sphingosine 1-phosphate.	transcription
59164	1	335897	5	NULL	NULL	0	NULL	p55TNFR		signaling of	stimulates					sphingomyelinase		neutral			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_14_9539_s_290	10092639	Signaling by the p55TNFR stimulates a neutral sphingomyelinase, which in turn generates ceramide and sphingosine.	transcription
59165	2	335897	5	NULL	NULL	0	NULL	statement 1			generates					ceramide					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_14_9539_s_290	10092639	Signaling by the p55TNFR stimulates a neutral sphingomyelinase, which in turn generates ceramide and sphingosine.	transcription
59166	3	335897	5	NULL	NULL	0	NULL	statement 1			generates					sphingosine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_14_9539_s_290	10092639	Signaling by the p55TNFR stimulates a neutral sphingomyelinase, which in turn generates ceramide and sphingosine.	transcription
79430	1	335897	6	NULL	NULL	0	NULL	p55TNFR	GP	signaling by	stimulates					sphingomyelinase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_14_9539_s_290	10092639	Signaling by the p55TNFR stimulates a neutral sphingomyelinase, which in turn generates ceramide and sphingosine.	transcription
79431	2	335897	6	NULL	NULL	0	NULL	sphingomyelinase	GP		generates					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_14_9539_s_290	10092639	Signaling by the p55TNFR stimulates a neutral sphingomyelinase, which in turn generates ceramide and sphingosine.	transcription
79432	3	335897	6	NULL	NULL	0	NULL	sphingomyelinase	GP		generates					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_14_9539_s_290	10092639	Signaling by the p55TNFR stimulates a neutral sphingomyelinase, which in turn generates ceramide and sphingosine.	transcription
59167	1	335898	5	NULL	NULL	0	NULL	ceramide			is formed in					ER					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_13_5055_s_227	16782891	It is still not clear whether the formation of ceramide in the ER depends directly on the availability of its substrate sphingosine or whether sphingosine activates specific ceramide synthase(s).	transcription
59168	2	335898	5	NULL	NULL	0	NULL	sphingosine			is a substrate of					ceramide					NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_13_5055_s_227	16782891	It is still not clear whether the formation of ceramide in the ER depends directly on the availability of its substrate sphingosine or whether sphingosine activates specific ceramide synthase(s).	transcription
59169	3	335898	5	NULL	NULL	0	NULL	statement 1			depends on		potentially;;directly			sphingosine		availability of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_13_5055_s_227	16782891	It is still not clear whether the formation of ceramide in the ER depends directly on the availability of its substrate sphingosine or whether sphingosine activates specific ceramide synthase(s).	transcription
59170	4	335898	5	NULL	NULL	0	NULL	sphingosine			activates		potentially			ceramide synthase		specific			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_13_5055_s_227	16782891	It is still not clear whether the formation of ceramide in the ER depends directly on the availability of its substrate sphingosine or whether sphingosine activates specific ceramide synthase(s).	transcription
59171	5	335898	5	NULL	NULL	0	NULL	statement 1			depends on		potentially;;directly			statement 4					NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_13_5055_s_227	16782891	It is still not clear whether the formation of ceramide in the ER depends directly on the availability of its substrate sphingosine or whether sphingosine activates specific ceramide synthase(s).	transcription
59172	1	335899	5	NULL	NULL	0	NULL	S1P			is dephosphorylated to					sphingosine					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34290_s_110	15180992	Dephosphorylation of S1P to sphingosine by SPP-1 has been associated with a large increase of ceramide levels resulting mainly from acylation of increased sphingosine by ceramide synthase ( ,  ).	transcription
59173	2	335899	5	NULL	NULL	0	NULL	SPP-1			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34290_s_110	15180992	Dephosphorylation of S1P to sphingosine by SPP-1 has been associated with a large increase of ceramide levels resulting mainly from acylation of increased sphingosine by ceramide synthase ( ,  ).	transcription
59197	3	335899	5	NULL	NULL	0	NULL	ceramide synthase			acylates					sphingosine		increased			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_33_34290_s_110	15180992	Dephosphorylation of S1P to sphingosine by SPP-1 has been associated with a large increase of ceramide levels resulting mainly from acylation of increased sphingosine by ceramide synthase ( ,  ).	transcription
59198	4	335899	5	NULL	NULL	0	NULL	statement 3			increases					ceramide		level of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34290_s_110	15180992	Dephosphorylation of S1P to sphingosine by SPP-1 has been associated with a large increase of ceramide levels resulting mainly from acylation of increased sphingosine by ceramide synthase ( ,  ).	transcription
59199	5	335899	5	NULL	NULL	0	NULL	statement 1			is associated with					statement 4					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34290_s_110	15180992	Dephosphorylation of S1P to sphingosine by SPP-1 has been associated with a large increase of ceramide levels resulting mainly from acylation of increased sphingosine by ceramide synthase ( ,  ).	transcription
79427	1	335899	6	NULL	NULL	0	NULL	S1P	GP		is converted to					sphingosine	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34290_s_110	15180992	Dephosphorylation of S1P to sphingosine by SPP-1 has been associated with a large increase of ceramide levels resulting mainly from acylation of increased sphingosine by ceramide synthase ( ,  ).	transcription
79428	2	335899	6	NULL	NULL	0	NULL	statement 1	Process		occurs by					SPP-1	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34290_s_110	15180992	Dephosphorylation of S1P to sphingosine by SPP-1 has been associated with a large increase of ceramide levels resulting mainly from acylation of increased sphingosine by ceramide synthase ( ,  ).	transcription
79429	3	335899	6	NULL	NULL	0	NULL	ceramide synthase	GP		acylates					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34290_s_110	15180992	Dephosphorylation of S1P to sphingosine by SPP-1 has been associated with a large increase of ceramide levels resulting mainly from acylation of increased sphingosine by ceramide synthase ( ,  ).	transcription
59215	1	335900	5	NULL	NULL	0	NULL	apoptosis			is mediated by					sphingosine					NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_154	9415703	Similarly, sphingosine-mediated apoptosis was unaffected by the ceramide synthase inhibitor fumonisin B1 (Table  3), indicating that acylation to ceramide did not contribute to the bioactivity of sphingosine.	transcription
59216	2	335900	5	NULL	NULL	0	NULL	fumonisin B1			does not affect					statement 1					NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_154	9415703	Similarly, sphingosine-mediated apoptosis was unaffected by the ceramide synthase inhibitor fumonisin B1 (Table  3), indicating that acylation to ceramide did not contribute to the bioactivity of sphingosine.	transcription
59217	3	335900	5	NULL	NULL	0	NULL	fumonisin B1			is an inhibitor of					ceramide synthase					NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_154	9415703	Similarly, sphingosine-mediated apoptosis was unaffected by the ceramide synthase inhibitor fumonisin B1 (Table  3), indicating that acylation to ceramide did not contribute to the bioactivity of sphingosine.	transcription
59218	4	335900	5	NULL	NULL	0	NULL	ceramide		acylation to	does not contribute to					sphingosine		bioactivity of			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_154	9415703	Similarly, sphingosine-mediated apoptosis was unaffected by the ceramide synthase inhibitor fumonisin B1 (Table  3), indicating that acylation to ceramide did not contribute to the bioactivity of sphingosine.	transcription
79424	1	335900	6	NULL	NULL	0	NULL	sphingosine	Chemical		mediates					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_154	9415703	Similarly, sphingosine-mediated apoptosis was unaffected by the ceramide synthase inhibitor fumonisin B1 (Table  3), indicating that acylation to ceramide did not contribute to the bioactivity of sphingosine.	transcription
79425	2	335900	6	NULL	NULL	0	NULL	fumonisin B1	Chemical		does not affect					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_154	9415703	Similarly, sphingosine-mediated apoptosis was unaffected by the ceramide synthase inhibitor fumonisin B1 (Table  3), indicating that acylation to ceramide did not contribute to the bioactivity of sphingosine.	transcription
79426	3	335900	6	NULL	NULL	0	NULL	ceramide	Chemical	acylation to	does not contribute to					sphingosine	Chemical	bioactivity of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_154	9415703	Similarly, sphingosine-mediated apoptosis was unaffected by the ceramide synthase inhibitor fumonisin B1 (Table  3), indicating that acylation to ceramide did not contribute to the bioactivity of sphingosine.	transcription
59219	1	335901	5	NULL	NULL	0	NULL	ceramide		initial increase in	preceded					sphingosine		increase in			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_147	10747891	The initial ceramide increase preceded that of sphingosine, suggesting that the increase in sphingosine might result from degradation of the ceramide formed upon Fas ligation.	transcription
59220	2	335901	5	NULL	NULL	0	NULL	ceramide			formed upon					Fas		ligation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_147	10747891	The initial ceramide increase preceded that of sphingosine, suggesting that the increase in sphingosine might result from degradation of the ceramide formed upon Fas ligation.	transcription
59221	3	335901	5	NULL	NULL	0	NULL	sphingosine		increase in	results from		might			ceramide		degradation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_147	10747891	The initial ceramide increase preceded that of sphingosine, suggesting that the increase in sphingosine might result from degradation of the ceramide formed upon Fas ligation.	transcription
59222	1	335902	5	NULL	NULL	0	NULL	ceramide			activates					cell death pathway					NULL	GST-P-positive cells in vitro	0	NULL	NULL	NULL	gw70_carcinogenesis_24_6_1077_s_210	12807752	Ceramide, sphingosine and an inhibitor of sphingosine kinase all activate a cell death pathway in such GST-P-positive cells  in vitro.	transcription
59223	2	335902	5	NULL	NULL	0	NULL	sphingosine			activates					cell death pathway					NULL	GST-P-positive cells in vitro	0	NULL	NULL	NULL	gw70_carcinogenesis_24_6_1077_s_210	12807752	Ceramide, sphingosine and an inhibitor of sphingosine kinase all activate a cell death pathway in such GST-P-positive cells  in vitro.	transcription
59224	3	335902	5	NULL	NULL	0	NULL	inhibitor of sphingosine kinase			activates					cell death pathway					NULL	GST-P-positive cells in vitro	0	NULL	NULL	NULL	gw70_carcinogenesis_24_6_1077_s_210	12807752	Ceramide, sphingosine and an inhibitor of sphingosine kinase all activate a cell death pathway in such GST-P-positive cells  in vitro.	transcription
79419	1	335902	6	NULL	NULL	0	NULL	ceramide	GP		activates					cell death pathway	Process				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_24_6_1077_s_210	12807752	Ceramide, sphingosine and an inhibitor of sphingosine kinase all activate a cell death pathway in such GST-P-positive cells  in vitro.	transcription
79420	2	335902	6	NULL	NULL	0	NULL	sphingosine	Chemical		activates					cell death pathway	Process				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_24_6_1077_s_210	12807752	Ceramide, sphingosine and an inhibitor of sphingosine kinase all activate a cell death pathway in such GST-P-positive cells  in vitro.	transcription
79421	3	335902	6	NULL	NULL	0	NULL	sphingosine kinase	GP	inhibitor of 	activates					cell death pathway	Process				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_24_6_1077_s_210	12807752	Ceramide, sphingosine and an inhibitor of sphingosine kinase all activate a cell death pathway in such GST-P-positive cells  in vitro.	transcription
59225	1	335903	5	NULL	NULL	0	NULL	sphingosine		exogenous	increases					ceramide		synthesis of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_943_s_8	15132973	When ceramide synthesis is increased through exogenous sphingosine or inhibition of sphingosine kinase, SRE-mediated gene transcription is increased.	transcription
59226	2	335903	5	NULL	NULL	0	NULL	sphingosine kinase		inhibition of	increases					ceramide		synthesis of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_943_s_8	15132973	When ceramide synthesis is increased through exogenous sphingosine or inhibition of sphingosine kinase, SRE-mediated gene transcription is increased.	transcription
59227	3	335903	5	NULL	NULL	0	NULL	SRE			mediates					gene transcription					NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_943_s_8	15132973	When ceramide synthesis is increased through exogenous sphingosine or inhibition of sphingosine kinase, SRE-mediated gene transcription is increased.	transcription
59228	4	335903	5	NULL	NULL	0	NULL	statement 1			increases					statement 3					NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_943_s_8	15132973	When ceramide synthesis is increased through exogenous sphingosine or inhibition of sphingosine kinase, SRE-mediated gene transcription is increased.	transcription
59229	5	335903	5	NULL	NULL	0	NULL	statement 2			increases					statement 3					NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_943_s_8	15132973	When ceramide synthesis is increased through exogenous sphingosine or inhibition of sphingosine kinase, SRE-mediated gene transcription is increased.	transcription
59230	1	335904	5	NULL	NULL	0	NULL	sphingosine			induce					apoptosis					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_50_50624_s_37	14522966	Whereas sphingosine induces apoptosis in various cell types ( ), sphingosine 1-phosphate antagonizes the apoptotic actions of ceramide ( ).	transcription
59231	2	335904	5	NULL	NULL	0	NULL	sphingosine 1-phosphate			antagonize					ceramide		apoptotic actions of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_50_50624_s_37	14522966	Whereas sphingosine induces apoptosis in various cell types ( ), sphingosine 1-phosphate antagonizes the apoptotic actions of ceramide ( ).	transcription
79416	1	335904	6	NULL	NULL	0	NULL	sphingosine	Chemical		induces					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_50_50624_s_37	14522966	Whereas sphingosine induces apoptosis in various cell types ( ), sphingosine 1-phosphate antagonizes the apoptotic actions of ceramide ( ).	transcription
79417	2	335904	6	NULL	NULL	0	NULL	sphingosine 1-phosphat	GP		suppresses					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_50_50624_s_37	14522966	Whereas sphingosine induces apoptosis in various cell types ( ), sphingosine 1-phosphate antagonizes the apoptotic actions of ceramide ( ).	transcription
79418	3	335904	6	NULL	NULL	0	NULL	ceramide	Chemical		induces					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_50_50624_s_37	14522966	Whereas sphingosine induces apoptosis in various cell types ( ), sphingosine 1-phosphate antagonizes the apoptotic actions of ceramide ( ).	transcription
59232	1	335905	5	NULL	NULL	0	NULL	TNF-alpha			stimulates					sphingosine kinase					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_3	11815603	TNF-alpha also stimulates sphingosine kinase, the enzyme that phosphorylates sphingosine to form sphingosine-1-phosphate (SPP), a further metabolite of ceramide.	transcription
59233	2	335905	5	NULL	NULL	0	NULL	sphingosine			is phosphorylated to					SPP					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_3	11815603	TNF-alpha also stimulates sphingosine kinase, the enzyme that phosphorylates sphingosine to form sphingosine-1-phosphate (SPP), a further metabolite of ceramide.	transcription
59234	3	335905	5	NULL	NULL	0	NULL	sphingosine kinase			catalyzes					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_3	11815603	TNF-alpha also stimulates sphingosine kinase, the enzyme that phosphorylates sphingosine to form sphingosine-1-phosphate (SPP), a further metabolite of ceramide.	transcription
59235	4	335905	5	NULL	NULL	0	NULL	SPP			is					sphingosine-1-phosphate					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_3	11815603	TNF-alpha also stimulates sphingosine kinase, the enzyme that phosphorylates sphingosine to form sphingosine-1-phosphate (SPP), a further metabolite of ceramide.	transcription
59236	5	335905	5	NULL	NULL	0	NULL	SPP			is a metabolite of					ceramide					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_3	11815603	TNF-alpha also stimulates sphingosine kinase, the enzyme that phosphorylates sphingosine to form sphingosine-1-phosphate (SPP), a further metabolite of ceramide.	transcription
79412	1	335905	6	NULL	NULL	0	NULL	TNF-alpha	GP		stimulates					sphingosine kinase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_3	11815603	TNF-alpha also stimulates sphingosine kinase, the enzyme that phosphorylates sphingosine to form sphingosine-1-phosphate (SPP), a further metabolite of ceramide.	transcription
79413	2	335905	6	NULL	NULL	0	NULL	sphingosine	GP		forms					sphingosine 1-phosphate	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_3	11815603	TNF-alpha also stimulates sphingosine kinase, the enzyme that phosphorylates sphingosine to form sphingosine-1-phosphate (SPP), a further metabolite of ceramide.	transcription
79414	3	335905	6	NULL	NULL	0	NULL	sphingosine kinase	GP		catalyzes					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_3	11815603	TNF-alpha also stimulates sphingosine kinase, the enzyme that phosphorylates sphingosine to form sphingosine-1-phosphate (SPP), a further metabolite of ceramide.	transcription
79415	4	335905	6	NULL	NULL	0	NULL	SPP	GP		is					sphingosine-1-phosphate	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_3	11815603	TNF-alpha also stimulates sphingosine kinase, the enzyme that phosphorylates sphingosine to form sphingosine-1-phosphate (SPP), a further metabolite of ceramide.	transcription
59237	1	335906	5	NULL	NULL	0	NULL	apoptosis			is induced by		directly			sphingosine					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_188	8626522	Consistent with the direct induction of apoptosis  by sphingosine described above, potentiation of ceramide-related  apoptosis by sphingosine was not stereoselective ( Table 3 ).	transcription
59238	2	335906	5	NULL	NULL	0	NULL	apoptosis			is related to					ceramide					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_188	8626522	Consistent with the direct induction of apoptosis  by sphingosine described above, potentiation of ceramide-related  apoptosis by sphingosine was not stereoselective ( Table 3 ).	transcription
59239	3	335906	5	NULL	NULL	0	NULL	sphingosine			potentiate					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_188	8626522	Consistent with the direct induction of apoptosis  by sphingosine described above, potentiation of ceramide-related  apoptosis by sphingosine was not stereoselective ( Table 3 ).	transcription
79411	1	335906	6	NULL	NULL	0	NULL	sphingosine	Chemical		induces					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_188	8626522	Consistent with the direct induction of apoptosis  by sphingosine described above, potentiation of ceramide-related  apoptosis by sphingosine was not stereoselective ( Table 3 ).	transcription
59240	1	335907	5	NULL	NULL	0	NULL	PLD			is activated by					ATP					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_8_1244_s_175	12177168	Therefore, it can be concluded that PLD activation by ATP is not mediated through the generation of ceramide or its further metabolism to sphingosine or sphingosine 1-phosphate.	transcription
59241	2	335907	5	NULL	NULL	0	NULL	statement 1			is not mediated through					ceramide		generation of			NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_8_1244_s_175	12177168	Therefore, it can be concluded that PLD activation by ATP is not mediated through the generation of ceramide or its further metabolism to sphingosine or sphingosine 1-phosphate.	transcription
59242	3	335907	5	NULL	NULL	0	NULL	ceramide			metabolized to					sphingosine					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_8_1244_s_175	12177168	Therefore, it can be concluded that PLD activation by ATP is not mediated through the generation of ceramide or its further metabolism to sphingosine or sphingosine 1-phosphate.	transcription
59243	4	335907	5	NULL	NULL	0	NULL	statement 1			is not mediated through					statement 3					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_8_1244_s_175	12177168	Therefore, it can be concluded that PLD activation by ATP is not mediated through the generation of ceramide or its further metabolism to sphingosine or sphingosine 1-phosphate.	transcription
59244	5	335907	5	NULL	NULL	0	NULL	ceramide			metabolized to					sphingosine 1-phosphate					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_8_1244_s_175	12177168	Therefore, it can be concluded that PLD activation by ATP is not mediated through the generation of ceramide or its further metabolism to sphingosine or sphingosine 1-phosphate.	transcription
59245	6	335907	5	NULL	NULL	0	NULL	statement 1			is not mediated through					statement 5					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_8_1244_s_175	12177168	Therefore, it can be concluded that PLD activation by ATP is not mediated through the generation of ceramide or its further metabolism to sphingosine or sphingosine 1-phosphate.	transcription
79409	1	335907	6	NULL	NULL	0	NULL	ATP	Chemical		activates					PLD	GP				NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_8_1244_s_175	12177168	Therefore, it can be concluded that PLD activation by ATP is not mediated through the generation of ceramide or its further metabolism to sphingosine or sphingosine 1-phosphate.	transcription
79410	2	335907	6	NULL	NULL	0	NULL	statement 1	Process		is not mediated through					ceramide	Chemical	generation of 			NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_8_1244_s_175	12177168	Therefore, it can be concluded that PLD activation by ATP is not mediated through the generation of ceramide or its further metabolism to sphingosine or sphingosine 1-phosphate.	transcription
59246	1	335908	5	NULL	NULL	0	NULL	sphingosine			is phosphorylated to					S1P					NULL		0	NULL	NULL	NULL	gw70_circulationres_98_11_1381_s_20	16675717	2 - 5    S1P is derived from the phosphorylation of sphingosine catalyzed by sphingosine kinase, sphingosine being from ceramide and ceramide from sphingomyelin, a constituent lipid of signaling microdomains of plasma membrane lipid rafts and caveolae.	transcription
59247	2	335908	5	NULL	NULL	0	NULL	sphingosine kinase			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw70_circulationres_98_11_1381_s_20	16675717	2 - 5    S1P is derived from the phosphorylation of sphingosine catalyzed by sphingosine kinase, sphingosine being from ceramide and ceramide from sphingomyelin, a constituent lipid of signaling microdomains of plasma membrane lipid rafts and caveolae.	transcription
59248	3	335908	5	NULL	NULL	0	NULL	sphingosine			is derived from					ceramide					NULL		0	NULL	NULL	NULL	gw70_circulationres_98_11_1381_s_20	16675717	2 - 5    S1P is derived from the phosphorylation of sphingosine catalyzed by sphingosine kinase, sphingosine being from ceramide and ceramide from sphingomyelin, a constituent lipid of signaling microdomains of plasma membrane lipid rafts and caveolae.	transcription
59249	4	335908	5	NULL	NULL	0	NULL	ceramide			is derived from					sphingomyelin					NULL		0	NULL	NULL	NULL	gw70_circulationres_98_11_1381_s_20	16675717	2 - 5    S1P is derived from the phosphorylation of sphingosine catalyzed by sphingosine kinase, sphingosine being from ceramide and ceramide from sphingomyelin, a constituent lipid of signaling microdomains of plasma membrane lipid rafts and caveolae.	transcription
59250	5	335908	5	NULL	NULL	0	NULL	sphingomyelin			is a type of					lipid					NULL		0	NULL	NULL	NULL	gw70_circulationres_98_11_1381_s_20	16675717	2 - 5    S1P is derived from the phosphorylation of sphingosine catalyzed by sphingosine kinase, sphingosine being from ceramide and ceramide from sphingomyelin, a constituent lipid of signaling microdomains of plasma membrane lipid rafts and caveolae.	transcription
79404	1	335908	6	NULL	NULL	0	NULL	sphingosine	Chemical	phosphorylation of	forms					S1P	GP				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_11_1381_s_20	16675717	2 - 5    S1P is derived from the phosphorylation of sphingosine catalyzed by sphingosine kinase, sphingosine being from ceramide and ceramide from sphingomyelin, a constituent lipid of signaling microdomains of plasma membrane lipid rafts and caveolae.	transcription
79405	2	335908	6	NULL	NULL	0	NULL	statement 1	Process		is catalyzed by					sphingosine kinase	GP				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_11_1381_s_20	16675717	2 - 5    S1P is derived from the phosphorylation of sphingosine catalyzed by sphingosine kinase, sphingosine being from ceramide and ceramide from sphingomyelin, a constituent lipid of signaling microdomains of plasma membrane lipid rafts and caveolae.	transcription
79406	3	335908	6	NULL	NULL	0	NULL	sphingosine	Chemical		is formed from					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_11_1381_s_20	16675717	2 - 5    S1P is derived from the phosphorylation of sphingosine catalyzed by sphingosine kinase, sphingosine being from ceramide and ceramide from sphingomyelin, a constituent lipid of signaling microdomains of plasma membrane lipid rafts and caveolae.	transcription
79407	4	335908	6	NULL	NULL	0	NULL	ceramide	Chemical		is formed from					sphingomyelin	Chemical				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_11_1381_s_20	16675717	2 - 5    S1P is derived from the phosphorylation of sphingosine catalyzed by sphingosine kinase, sphingosine being from ceramide and ceramide from sphingomyelin, a constituent lipid of signaling microdomains of plasma membrane lipid rafts and caveolae.	transcription
79408	5	335908	6	NULL	NULL	0	NULL	sphingomyelin	Chemical		is a type of					lipid molecule	Chemical				NULL		0	NULL	NULL	NULL	gw70_circulationres_98_11_1381_s_20	16675717	2 - 5    S1P is derived from the phosphorylation of sphingosine catalyzed by sphingosine kinase, sphingosine being from ceramide and ceramide from sphingomyelin, a constituent lipid of signaling microdomains of plasma membrane lipid rafts and caveolae.	transcription
59251	1	335909	5	NULL	NULL	0	NULL	sphingosine			does not activate					phospholipase D		activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_10	7592842	Sphingosine did not activate  phospholipase D activity significantly after 10 min.  C -ceramide stimulated the conversion of exogenous  [ H]sphingosine 1-phosphate to sphingosine and  ceramide in fibroblasts.	transcription
59252	2	335909	5	NULL	NULL	0	NULL	sphingosine 1-phosphate		exogenous	is converted to					sphingosine					NULL	fibroblasts	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_10	7592842	Sphingosine did not activate  phospholipase D activity significantly after 10 min.  C -ceramide stimulated the conversion of exogenous  [ H]sphingosine 1-phosphate to sphingosine and  ceramide in fibroblasts.	transcription
59253	3	335909	5	NULL	NULL	0	NULL	sphingosine 1-phosphate		exogenous	is converted to					ceramide					NULL	fibroblasts	0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_10	7592842	Sphingosine did not activate  phospholipase D activity significantly after 10 min.  C -ceramide stimulated the conversion of exogenous  [ H]sphingosine 1-phosphate to sphingosine and  ceramide in fibroblasts.	transcription
59254	4	335909	5	NULL	NULL	0	NULL	C -ceramide			stimulates					statement 2					NULL	fibroblasts	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_10	7592842	Sphingosine did not activate  phospholipase D activity significantly after 10 min.  C -ceramide stimulated the conversion of exogenous  [ H]sphingosine 1-phosphate to sphingosine and  ceramide in fibroblasts.	transcription
59255	5	335909	5	NULL	NULL	0	NULL	C -ceramide			stimulates					statement 3					NULL	fibroblasts	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_10	7592842	Sphingosine did not activate  phospholipase D activity significantly after 10 min.  C -ceramide stimulated the conversion of exogenous  [ H]sphingosine 1-phosphate to sphingosine and  ceramide in fibroblasts.	transcription
79399	1	335909	6	NULL	NULL	0	NULL	sphingosine	Chemical		does not activate					phospholipase D	GP	activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_10	7592842	Sphingosine did not activate  phospholipase D activity significantly after 10 min.  C -ceramide stimulated the conversion of exogenous  [ H]sphingosine 1-phosphate to sphingosine and  ceramide in fibroblasts.	transcription
79400	2	335909	6	NULL	NULL	0	NULL	sphingosine 1-phosphate	GP		is converted to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_10	7592842	Sphingosine did not activate  phospholipase D activity significantly after 10 min.  C -ceramide stimulated the conversion of exogenous  [ H]sphingosine 1-phosphate to sphingosine and  ceramide in fibroblasts.	transcription
79401	3	335909	6	NULL	NULL	0	NULL	sphingosine 1-phosphate	Chemical		is converted to					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_10	7592842	Sphingosine did not activate  phospholipase D activity significantly after 10 min.  C -ceramide stimulated the conversion of exogenous  [ H]sphingosine 1-phosphate to sphingosine and  ceramide in fibroblasts.	transcription
79402	4	335909	6	NULL	NULL	0	NULL	ceramide	Chemical		catalyzes					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_10	7592842	Sphingosine did not activate  phospholipase D activity significantly after 10 min.  C -ceramide stimulated the conversion of exogenous  [ H]sphingosine 1-phosphate to sphingosine and  ceramide in fibroblasts.	transcription
79403	5	335909	6	NULL	NULL	0	NULL	ceramide	GP		catalyzes					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_10	7592842	Sphingosine did not activate  phospholipase D activity significantly after 10 min.  C -ceramide stimulated the conversion of exogenous  [ H]sphingosine 1-phosphate to sphingosine and  ceramide in fibroblasts.	transcription
59256	1	335910	5	NULL	NULL	0	NULL	sphingosine-1 phosphate			is a type of					lipid					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_32_22532_s_219	10428830	Incidentally, another lipid that was shown to counteract the effects of ceramide and to inhibit CD95-mediated apoptosis, sphingosine-1 phosphate, was also shown to be active in Jurkat T cells ( 17,  62).	transcription
59257	2	335910	5	NULL	NULL	0	NULL	sphingosine-1 phosphate			counteracts					ceramide		effects of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_32_22532_s_219	10428830	Incidentally, another lipid that was shown to counteract the effects of ceramide and to inhibit CD95-mediated apoptosis, sphingosine-1 phosphate, was also shown to be active in Jurkat T cells ( 17,  62).	transcription
59258	3	335910	5	NULL	NULL	0	NULL	apoptosis			is mediated by					CD95					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_32_22532_s_219	10428830	Incidentally, another lipid that was shown to counteract the effects of ceramide and to inhibit CD95-mediated apoptosis, sphingosine-1 phosphate, was also shown to be active in Jurkat T cells ( 17,  62).	transcription
59259	4	335910	5	NULL	NULL	0	NULL	sphingosine-1 phosphate			inhibits					statement 4					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_32_22532_s_219	10428830	Incidentally, another lipid that was shown to counteract the effects of ceramide and to inhibit CD95-mediated apoptosis, sphingosine-1 phosphate, was also shown to be active in Jurkat T cells ( 17,  62).	transcription
59260	5	335910	5	NULL	NULL	0	NULL	sphingosine-1 phosphate			active in					Jurkat T cells					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_32_22532_s_219	10428830	Incidentally, another lipid that was shown to counteract the effects of ceramide and to inhibit CD95-mediated apoptosis, sphingosine-1 phosphate, was also shown to be active in Jurkat T cells ( 17,  62).	transcription
59261	1	335912	5	NULL	NULL	0	NULL	ceramide			deamidated to					sphingosine					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_193	14702348	Effect of Ceramide Metabolism on the Toxin-induced Hemolysis of Sheep Erythrocytes -- Ceramide is known to be deamidated to sphingosine by ceramidase.	transcription
59262	2	335912	5	NULL	NULL	0	NULL	ceramidase			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_193	14702348	Effect of Ceramide Metabolism on the Toxin-induced Hemolysis of Sheep Erythrocytes -- Ceramide is known to be deamidated to sphingosine by ceramidase.	transcription
59263	3	335912	5	NULL	NULL	0	NULL	erythrocytes 		sheep	undergoes					hemolysis					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_193	14702348	Effect of Ceramide Metabolism on the Toxin-induced Hemolysis of Sheep Erythrocytes -- Ceramide is known to be deamidated to sphingosine by ceramidase.	transcription
59264	4	335912	5	NULL	NULL	0	NULL	toxin			induce					statement 3					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_193	14702348	Effect of Ceramide Metabolism on the Toxin-induced Hemolysis of Sheep Erythrocytes -- Ceramide is known to be deamidated to sphingosine by ceramidase.	transcription
59265	5	335912	5	NULL	NULL	0	NULL	ceramide		metabolism of	effects		potentially			statement 3					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_193	14702348	Effect of Ceramide Metabolism on the Toxin-induced Hemolysis of Sheep Erythrocytes -- Ceramide is known to be deamidated to sphingosine by ceramidase.	transcription
79397	1	335912	6	NULL	NULL	0	NULL	ceramide	Chemical		is deaminated to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_193	14702348	Effect of Ceramide Metabolism on the Toxin-induced Hemolysis of Sheep Erythrocytes -- Ceramide is known to be deamidated to sphingosine by ceramidase.	transcription
79398	2	335912	6	NULL	NULL	0	NULL	statement 1	Process		is catalyzed by					ceramidase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_193	14702348	Effect of Ceramide Metabolism on the Toxin-induced Hemolysis of Sheep Erythrocytes -- Ceramide is known to be deamidated to sphingosine by ceramidase.	transcription
59266	1	335913	5	NULL	NULL	0	NULL	ceramide			deamidated to					sphingosine					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_212	14702348	These results suggested that  N-oleoylethanolamine specifically blocked the toxin-stimulated deamidation of ceramide to sphingosine, resulting in the accumulation of ceramide.	transcription
59267	2	335913	5	NULL	NULL	0	NULL	statement 1			is stimulated by					toxin					NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_212	14702348	These results suggested that  N-oleoylethanolamine specifically blocked the toxin-stimulated deamidation of ceramide to sphingosine, resulting in the accumulation of ceramide.	transcription
59268	3	335913	5	NULL	NULL	0	NULL	N-oleoylethanolamine			blocks		specifically			statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_212	14702348	These results suggested that  N-oleoylethanolamine specifically blocked the toxin-stimulated deamidation of ceramide to sphingosine, resulting in the accumulation of ceramide.	transcription
59269	4	335913	5	NULL	NULL	0	NULL	statement 3			accumulates					ceramide					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_212	14702348	These results suggested that  N-oleoylethanolamine specifically blocked the toxin-stimulated deamidation of ceramide to sphingosine, resulting in the accumulation of ceramide.	transcription
79395	1	335913	6	NULL	NULL	0	NULL	ceramide	Chemical		is deaminated to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_212	14702348	These results suggested that  N-oleoylethanolamine specifically blocked the toxin-stimulated deamidation of ceramide to sphingosine, resulting in the accumulation of ceramide.	transcription
79396	2	335913	6	NULL	NULL	0	NULL	N-oleoylethanolamine	Chemical		blocks					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_212	14702348	These results suggested that  N-oleoylethanolamine specifically blocked the toxin-stimulated deamidation of ceramide to sphingosine, resulting in the accumulation of ceramide.	transcription
59270	1	335914	5	NULL	NULL	0	NULL	dihydrosphingosine			N-acylated to					ceramide					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_10	12424251	The formation of ceramide resulting from the  N-acylation of dihydrosphingosine or sphingosine by ceramide synthase is inhibited by the fungal toxin fumonisin B1.	transcription
59271	2	335914	5	NULL	NULL	0	NULL	ceramide synthase			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_10	12424251	The formation of ceramide resulting from the  N-acylation of dihydrosphingosine or sphingosine by ceramide synthase is inhibited by the fungal toxin fumonisin B1.	transcription
59272	3	335914	5	NULL	NULL	0	NULL	sphingosine			N-acylated to					ceramide					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_10	12424251	The formation of ceramide resulting from the  N-acylation of dihydrosphingosine or sphingosine by ceramide synthase is inhibited by the fungal toxin fumonisin B1.	transcription
59273	4	335914	5	NULL	NULL	0	NULL	ceramide synthase			catalyzes					statement 3					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_10	12424251	The formation of ceramide resulting from the  N-acylation of dihydrosphingosine or sphingosine by ceramide synthase is inhibited by the fungal toxin fumonisin B1.	transcription
59274	5	335914	5	NULL	NULL	0	NULL	fumonisin B1			inhibits					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_10	12424251	The formation of ceramide resulting from the  N-acylation of dihydrosphingosine or sphingosine by ceramide synthase is inhibited by the fungal toxin fumonisin B1.	transcription
59275	6	335914	5	NULL	NULL	0	NULL	fumonisin B1			inhibits					statement 3					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_10	12424251	The formation of ceramide resulting from the  N-acylation of dihydrosphingosine or sphingosine by ceramide synthase is inhibited by the fungal toxin fumonisin B1.	transcription
59276	7	335914	5	NULL	NULL	0	NULL	fumonisin B1			is a type of					fungal toxin					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_10	12424251	The formation of ceramide resulting from the  N-acylation of dihydrosphingosine or sphingosine by ceramide synthase is inhibited by the fungal toxin fumonisin B1.	transcription
59277	1	335915	5	NULL	NULL	0	NULL	sphingosine			is converted to					dihydroceramide					NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_253	15772421	The pathways  discussed in this study include the de novo pathway involving the conversion of sphinganine  to dihydroceramide or sphingosine to ceramide catalyzed by ceramide synthase	transcription
59278	2	335915	5	NULL	NULL	0	NULL	ceramide synthase			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_253	15772421	The pathways  discussed in this study include the de novo pathway involving the conversion of sphinganine  to dihydroceramide or sphingosine to ceramide catalyzed by ceramide synthase	transcription
59279	3	335915	5	NULL	NULL	0	NULL	sphingosine			is converted to					ceramide					NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_253	15772421	The pathways  discussed in this study include the de novo pathway involving the conversion of sphinganine  to dihydroceramide or sphingosine to ceramide catalyzed by ceramide synthase	transcription
59280	4	335915	5	NULL	NULL	0	NULL	ceramide synthase			catalyzes					statement 3					NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_253	15772421	The pathways  discussed in this study include the de novo pathway involving the conversion of sphinganine  to dihydroceramide or sphingosine to ceramide catalyzed by ceramide synthase	transcription
79391	1	335915	6	NULL	NULL	0	NULL	sphinganine	Chemical		is converted to					dihydroceramide	Chemical				NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_253	15772421	The pathways  discussed in this study include the de novo pathway involving the conversion of sphinganine  to dihydroceramide or sphingosine to ceramide catalyzed by ceramide synthase	transcription
79392	2	335915	6	NULL	NULL	0	NULL	sphingosine	Chemical		is converted to					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_253	15772421	The pathways  discussed in this study include the de novo pathway involving the conversion of sphinganine  to dihydroceramide or sphingosine to ceramide catalyzed by ceramide synthase	transcription
79393	3	335915	6	NULL	NULL	0	NULL	ceramide synthase	GP		catalyzes					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_253	15772421	The pathways  discussed in this study include the de novo pathway involving the conversion of sphinganine  to dihydroceramide or sphingosine to ceramide catalyzed by ceramide synthase	transcription
79394	4	335915	6	NULL	NULL	0	NULL	ceramide synthase	GP		catalyzes					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_253	15772421	The pathways  discussed in this study include the de novo pathway involving the conversion of sphinganine  to dihydroceramide or sphingosine to ceramide catalyzed by ceramide synthase	transcription
59354	1	335916	5	NULL	NULL	0	NULL	sphinganine			N-acylated to					dihydroceramide					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_33_20373_s_113	9252342	Ceramide synthase catalyzes the  N-acylation of sphinganine or sphingosine with a long chain fatty acyl-CoA to form dihydroceramide or ceramide.	transcription
59355	2	335916	5	NULL	NULL	0	NULL	sphinganine			N-acylated to					ceramide					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_33_20373_s_113	9252342	Ceramide synthase catalyzes the  N-acylation of sphinganine or sphingosine with a long chain fatty acyl-CoA to form dihydroceramide or ceramide.	transcription
59356	3	335916	5	NULL	NULL	0	NULL	statement 1			is an alternative to					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_33_20373_s_113	9252342	Ceramide synthase catalyzes the  N-acylation of sphinganine or sphingosine with a long chain fatty acyl-CoA to form dihydroceramide or ceramide.	transcription
59357	4	335916	5	NULL	NULL	0	NULL	ceramide synthase			catalyzes					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_33_20373_s_113	9252342	Ceramide synthase catalyzes the  N-acylation of sphinganine or sphingosine with a long chain fatty acyl-CoA to form dihydroceramide or ceramide.	transcription
59358	5	335916	5	NULL	NULL	0	NULL	ceramide synthase			catalyzes					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_33_20373_s_113	9252342	Ceramide synthase catalyzes the  N-acylation of sphinganine or sphingosine with a long chain fatty acyl-CoA to form dihydroceramide or ceramide.	transcription
59359	6	335916	5	NULL	NULL	0	NULL	sphingosine			contains					long chain fatty acyl-CoA					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_33_20373_s_113	9252342	Ceramide synthase catalyzes the  N-acylation of sphinganine or sphingosine with a long chain fatty acyl-CoA to form dihydroceramide or ceramide.	transcription
59360	7	335916	5	NULL	NULL	0	NULL	sphingosine			N-acylated to					dihydroceramide					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_33_20373_s_113	9252342	Ceramide synthase catalyzes the  N-acylation of sphinganine or sphingosine with a long chain fatty acyl-CoA to form dihydroceramide or ceramide.	transcription
59362	8	335916	5	NULL	NULL	0	NULL	sphingosine			N-acylated to					ceramide					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_33_20373_s_113	9252342	Ceramide synthase catalyzes the  N-acylation of sphinganine or sphingosine with a long chain fatty acyl-CoA to form dihydroceramide or ceramide.	transcription
59363	9	335916	5	NULL	NULL	0	NULL	statement 7			is an alternative to					statement 8					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_33_20373_s_113	9252342	Ceramide synthase catalyzes the  N-acylation of sphinganine or sphingosine with a long chain fatty acyl-CoA to form dihydroceramide or ceramide.	transcription
59364	10	335916	5	NULL	NULL	0	NULL	ceramide synthase \t			catalyzes					statement 7					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_33_20373_s_113	9252342	Ceramide synthase catalyzes the  N-acylation of sphinganine or sphingosine with a long chain fatty acyl-CoA to form dihydroceramide or ceramide.	transcription
59365	11	335916	5	NULL	NULL	0	NULL	ceramide synthase			catalyzes					statement 8					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_33_20373_s_113	9252342	Ceramide synthase catalyzes the  N-acylation of sphinganine or sphingosine with a long chain fatty acyl-CoA to form dihydroceramide or ceramide.	transcription
79388	1	335916	6	NULL	NULL	0	NULL	sphinganine	Chemical		forms					dihydroceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_33_20373_s_113	9252342	Ceramide synthase catalyzes the  N-acylation of sphinganine or sphingosine with a long chain fatty acyl-CoA to form dihydroceramide or ceramide.	transcription
79389	2	335916	6	NULL	NULL	0	NULL	Ceramide synthase	GP		catalyzes					sphingosine	GP	N-acylation of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_33_20373_s_113	9252342	Ceramide synthase catalyzes the  N-acylation of sphinganine or sphingosine with a long chain fatty acyl-CoA to form dihydroceramide or ceramide.	transcription
79390	3	335916	6	NULL	NULL	0	NULL	ceramide synthase	GP		catalyzes					sphinganine	GP	N-acylation of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_33_20373_s_113	9252342	Ceramide synthase catalyzes the  N-acylation of sphinganine or sphingosine with a long chain fatty acyl-CoA to form dihydroceramide or ceramide.	transcription
59281	1	335917	5	NULL	NULL	0	NULL	apoptosis			is mediated by					sphingosine					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_261	10747891	Sphingosine- and Ceramide-mediated Apoptosis Is Mitochondria-dependent-- Mitochondrial dysfunction appears to be important in ceramide signaling of apoptosis ( 77).	transcription
59282	2	335917	5	NULL	NULL	0	NULL	statement 1			is dependent on					mitochondria					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_261	10747891	Sphingosine- and Ceramide-mediated Apoptosis Is Mitochondria-dependent-- Mitochondrial dysfunction appears to be important in ceramide signaling of apoptosis ( 77).	transcription
59283	3	335917	5	NULL	NULL	0	NULL	apoptosis			is mediated by					ceramide					NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_261	10747891	Sphingosine- and Ceramide-mediated Apoptosis Is Mitochondria-dependent-- Mitochondrial dysfunction appears to be important in ceramide signaling of apoptosis ( 77).	transcription
59284	4	335917	5	NULL	NULL	0	NULL	statement 3			is dependent on					mitochondria					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_261	10747891	Sphingosine- and Ceramide-mediated Apoptosis Is Mitochondria-dependent-- Mitochondrial dysfunction appears to be important in ceramide signaling of apoptosis ( 77).	transcription
59385	5	335917	5	NULL	NULL	0	NULL	mitochondria		dysfunction of	is important for		may be			statement 3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_261	10747891	Sphingosine- and Ceramide-mediated Apoptosis Is Mitochondria-dependent-- Mitochondrial dysfunction appears to be important in ceramide signaling of apoptosis ( 77).	transcription
79384	1	335917	6	NULL	NULL	0	NULL	sphingosine	Chemical		mediates					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_261	10747891	Sphingosine- and Ceramide-mediated Apoptosis Is Mitochondria-dependent-- Mitochondrial dysfunction appears to be important in ceramide signaling of apoptosis ( 77).	transcription
79385	2	335917	6	NULL	NULL	0	NULL	ceramide	Chemical		mediates					apoptosis	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_261	10747891	Sphingosine- and Ceramide-mediated Apoptosis Is Mitochondria-dependent-- Mitochondrial dysfunction appears to be important in ceramide signaling of apoptosis ( 77).	transcription
79386	3	335917	6	NULL	NULL	0	NULL	statement 1	Process		is dependent on					mitochondria	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_261	10747891	Sphingosine- and Ceramide-mediated Apoptosis Is Mitochondria-dependent-- Mitochondrial dysfunction appears to be important in ceramide signaling of apoptosis ( 77).	transcription
79387	4	335917	6	NULL	NULL	0	NULL	statement 2	Process		is dependent on					mitochondria	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_261	10747891	Sphingosine- and Ceramide-mediated Apoptosis Is Mitochondria-dependent-- Mitochondrial dysfunction appears to be important in ceramide signaling of apoptosis ( 77).	transcription
59386	1	335918	5	NULL	NULL	0	NULL	FB1			inhibits					ceramide synthase					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_18_12367_s_26	10212208	FB1 inhibits ceramide synthase, which alters sphinganine:sphingosine ratios ( 16,  17) and inhibits the synthesis of ceramide.	transcription
59387	2	335918	5	NULL	NULL	0	NULL	ceramide synthase			alters					sphinganine:sphingosine ratios					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_18_12367_s_26	10212208	FB1 inhibits ceramide synthase, which alters sphinganine:sphingosine ratios ( 16,  17) and inhibits the synthesis of ceramide.	transcription
59388	3	335918	5	NULL	NULL	0	NULL	FB1			inhibits					ceramide		synthesis of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_18_12367_s_26	10212208	FB1 inhibits ceramide synthase, which alters sphinganine:sphingosine ratios ( 16,  17) and inhibits the synthesis of ceramide.	transcription
79383	1	335918	6	NULL	NULL	0	NULL	FB1	Chemical		inhibits					ceramide synthase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_18_12367_s_26	10212208	FB1 inhibits ceramide synthase, which alters sphinganine:sphingosine ratios ( 16,  17) and inhibits the synthesis of ceramide.	transcription
59389	1	335919	5	NULL	NULL	0	NULL	sphingosine 1-phosphate			is a catabolite of					ceramide					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21121_s_17	10409665	On the other hand, ceramide catabolites, such as sphingosine 1-phosphate, stimulate cell growth and suppress ceramide-mediated cell death ( 5).	transcription
59390	2	335919	5	NULL	NULL	0	NULL	sphingosine 1-phosphate			stimulates					cell growth					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21121_s_17	10409665	On the other hand, ceramide catabolites, such as sphingosine 1-phosphate, stimulate cell growth and suppress ceramide-mediated cell death ( 5).	transcription
59391	3	335919	5	NULL	NULL	0	NULL	ceramide			mediates					cell death					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21121_s_17	10409665	On the other hand, ceramide catabolites, such as sphingosine 1-phosphate, stimulate cell growth and suppress ceramide-mediated cell death ( 5).	transcription
59392	4	335919	5	NULL	NULL	0	NULL	sphingosine 1-phosphate			supress					statement 3					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21121_s_17	10409665	On the other hand, ceramide catabolites, such as sphingosine 1-phosphate, stimulate cell growth and suppress ceramide-mediated cell death ( 5).	transcription
79380	1	335919	6	NULL	NULL	0	NULL	sphingosine 1-phosphate	Chemical		stimulates					cell growth	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21121_s_17	10409665	On the other hand, ceramide catabolites, such as sphingosine 1-phosphate, stimulate cell growth and suppress ceramide-mediated cell death ( 5).	transcription
79381	2	335919	6	NULL	NULL	NULL	NULL	sphingosine 1-phosphate	GP		suppresses					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_30_21121_s_17	10409665	On the other hand, ceramide catabolites, such as sphingosine 1-phosphate, stimulate cell growth and suppress ceramide-mediated cell death ( 5).	transcription
79382	3	335919	6	NULL	NULL	0	NULL	ceramide	Chemical		mediates					cell death	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_21121_s_17	10409665	On the other hand, ceramide catabolites, such as sphingosine 1-phosphate, stimulate cell growth and suppress ceramide-mediated cell death ( 5).	transcription
59393	1	335920	5	NULL	NULL	0	NULL	fumonisin B1			is an inhibitor of					ceramide synthase					NULL		0	NULL	NULL	NULL	abs-batch0530-0539_j-bioenerg-biomembr_37_4_16167178_s_7	16167178	The ceramide synthase inhibitor, fumonisin B1 failed to prevent sphingosine  metabolism to ceramide and actually increased it.	transcription
59394	2	335920	5	NULL	NULL	0	NULL	sphingosine			metabolized to					ceramide					NULL		0	NULL	NULL	NULL	abs-batch0530-0539_j-bioenerg-biomembr_37_4_16167178_s_7	16167178	The ceramide synthase inhibitor, fumonisin B1 failed to prevent sphingosine  metabolism to ceramide and actually increased it.	transcription
59395	3	335920	5	NULL	NULL	0	NULL	fumonisin B1			does not prevent					statement 2					NULL		0	NULL	NULL	NULL	abs-batch0530-0539_j-bioenerg-biomembr_37_4_16167178_s_7	16167178	The ceramide synthase inhibitor, fumonisin B1 failed to prevent sphingosine  metabolism to ceramide and actually increased it.	transcription
59396	4	335920	5	NULL	NULL	0	NULL	fumonisin B1			increases					statement 2					NULL		0	NULL	NULL	NULL	abs-batch0530-0539_j-bioenerg-biomembr_37_4_16167178_s_7	16167178	The ceramide synthase inhibitor, fumonisin B1 failed to prevent sphingosine  metabolism to ceramide and actually increased it.	transcription
79377	1	335920	6	NULL	NULL	0	NULL	sphingosine	Chemical		is converted to					ceramide	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_j-bioenerg-biomembr_37_4_16167178_s_7	16167178	The ceramide synthase inhibitor, fumonisin B1 failed to prevent sphingosine  metabolism to ceramide and actually increased it.	transcription
79378	2	335920	6	NULL	NULL	0	NULL	fumonisin B1	Chemical		prevents					statement 1	Process				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_j-bioenerg-biomembr_37_4_16167178_s_7	16167178	The ceramide synthase inhibitor, fumonisin B1 failed to prevent sphingosine  metabolism to ceramide and actually increased it.	transcription
79379	3	335920	6	NULL	NULL	0	NULL	fumonisin B1	Chemical		is a type of					ceramide synthase inhibitor	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0530-0539_j-bioenerg-biomembr_37_4_16167178_s_7	16167178	The ceramide synthase inhibitor, fumonisin B1 failed to prevent sphingosine  metabolism to ceramide and actually increased it.	transcription
59397	1	335921	5	NULL	NULL	0	NULL	C2-Cer			induces					ceramides		accumulation of;;endogenous;;long chain			NULL	HT-29 cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_279_18_18384_s_144	14970205	From these results we concluded that C2-Cer induces an accumulation of endogenous long chain ceramides in HT-29 cells, and this accumulation is dependent on the recycling of the sphingosine moiety and the activity of ceramide synthase.	transcription
59398	2	335921	5	NULL	NULL	0	NULL	ceramides		accumulation of;;endogenous;;long chain	is dependent on					sphingosine moiety		recycling of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_18_18384_s_144	14970205	From these results we concluded that C2-Cer induces an accumulation of endogenous long chain ceramides in HT-29 cells, and this accumulation is dependent on the recycling of the sphingosine moiety and the activity of ceramide synthase.	transcription
59399	3	335921	5	NULL	NULL	0	NULL	ceramides		accumulation of;;endogenous;;long chain	is dependent on					ceramide synthase		activity of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_18_18384_s_144	14970205	From these results we concluded that C2-Cer induces an accumulation of endogenous long chain ceramides in HT-29 cells, and this accumulation is dependent on the recycling of the sphingosine moiety and the activity of ceramide synthase.	transcription
79374	1	335921	6	NULL	NULL	0	NULL	C2-cer	Chemical		induces					long chain ceramides	Chemical	accumulation of;; endogenous			NULL	HT-29 cells	0	NULL	NULL	NULL	gw70_jbiolchem_279_18_18384_s_144	14970205	From these results we concluded that C2-Cer induces an accumulation of endogenous long chain ceramides in HT-29 cells, and this accumulation is dependent on the recycling of the sphingosine moiety and the activity of ceramide synthase.	transcription
79375	2	335921	6	NULL	NULL	0	NULL	statement 1	Process		is dependent on					ceramide synthase	GP	activity of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_18_18384_s_144	14970205	From these results we concluded that C2-Cer induces an accumulation of endogenous long chain ceramides in HT-29 cells, and this accumulation is dependent on the recycling of the sphingosine moiety and the activity of ceramide synthase.	transcription
79376	3	335921	6	NULL	NULL	0	NULL	statement 1	Process		is dependent on					sphingosine	Chemical	recycling of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_18_18384_s_144	14970205	From these results we concluded that C2-Cer induces an accumulation of endogenous long chain ceramides in HT-29 cells, and this accumulation is dependent on the recycling of the sphingosine moiety and the activity of ceramide synthase.	transcription
59400	1	335922	5	NULL	NULL	0	NULL	sphingosine			is converted to					ceramide					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_3_1255_s_74	8576106	However, Fumonisin B1, which  inhibits the conversion of sphingosine to ceramide( 24) , did  not inhibit the effect of exogenously added sphingosine on the ISP-1  action ( 14) , suggesting that ceramide is not the downstream  effector and that sphingosine derivatives with a free amino group such  as sphingosine and sphingosine 1-phosphate are possible candidates.	transcription
59401	2	335922	5	NULL	NULL	0	NULL	Fumonisin B1			inhibits					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_3_1255_s_74	8576106	However, Fumonisin B1, which  inhibits the conversion of sphingosine to ceramide( 24) , did  not inhibit the effect of exogenously added sphingosine on the ISP-1  action ( 14) , suggesting that ceramide is not the downstream  effector and that sphingosine derivatives with a free amino group such  as sphingosine and sphingosine 1-phosphate are possible candidates.	transcription
79372	1	335922	6	NULL	NULL	0	NULL	sphingosine	Chemical		is converted to					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_3_1255_s_74	8576106	However, Fumonisin B1, which  inhibits the conversion of sphingosine to ceramide( 24) , did  not inhibit the effect of exogenously added sphingosine on the ISP-1  action ( 14) , suggesting that ceramide is not the downstream  effector and that sphingosine derivatives with a free amino group such  as sphingosine and sphingosine 1-phosphate are possible candidates.	transcription
79373	2	335922	6	NULL	NULL	0	NULL	Fumonisin B1	Chemical		inhibits					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_3_1255_s_74	8576106	However, Fumonisin B1, which  inhibits the conversion of sphingosine to ceramide( 24) , did  not inhibit the effect of exogenously added sphingosine on the ISP-1  action ( 14) , suggesting that ceramide is not the downstream  effector and that sphingosine derivatives with a free amino group such  as sphingosine and sphingosine 1-phosphate are possible candidates.	transcription
59402	1	335923	5	NULL	NULL	0	NULL	sphingosine			N-acylated to					ceramide					NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_78	12135749	Because sphingosine could be converted to ceramide by  N-acylation and ceramide could induce c-jun expression, we used fumonisin B1, an inhibitor of ceramide synthase, to investigate whether sphingosine itself induced c-jun expression.	transcription
59403	2	335923	5	NULL	NULL	0	NULL	ceramide			induce					c-jun		expression of			NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_78	12135749	Because sphingosine could be converted to ceramide by  N-acylation and ceramide could induce c-jun expression, we used fumonisin B1, an inhibitor of ceramide synthase, to investigate whether sphingosine itself induced c-jun expression.	transcription
59404	3	335923	5	NULL	NULL	0	NULL	fumonisin B1			is an inhibitor of					ceramide synthase					NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_78	12135749	Because sphingosine could be converted to ceramide by  N-acylation and ceramide could induce c-jun expression, we used fumonisin B1, an inhibitor of ceramide synthase, to investigate whether sphingosine itself induced c-jun expression.	transcription
59405	4	335923	5	NULL	NULL	0	NULL	sphingosine			induce		potentially			c-jun		expression of			NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_78	12135749	Because sphingosine could be converted to ceramide by  N-acylation and ceramide could induce c-jun expression, we used fumonisin B1, an inhibitor of ceramide synthase, to investigate whether sphingosine itself induced c-jun expression.	transcription
79369	1	335923	6	NULL	NULL	0	NULL	sphingosine	Chemical		is converted to					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_78	12135749	Because sphingosine could be converted to ceramide by  N-acylation and ceramide could induce c-jun expression, we used fumonisin B1, an inhibitor of ceramide synthase, to investigate whether sphingosine itself induced c-jun expression.	transcription
79370	2	335923	6	NULL	NULL	0	NULL	statement 1	Process		occurs by					N-acylation	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_78	12135749	Because sphingosine could be converted to ceramide by  N-acylation and ceramide could induce c-jun expression, we used fumonisin B1, an inhibitor of ceramide synthase, to investigate whether sphingosine itself induced c-jun expression.	transcription
79371	3	335923	6	NULL	NULL	0	NULL	ceramide	Chemical		induces					c-jun	GP	expression of			NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_78	12135749	Because sphingosine could be converted to ceramide by  N-acylation and ceramide could induce c-jun expression, we used fumonisin B1, an inhibitor of ceramide synthase, to investigate whether sphingosine itself induced c-jun expression.	transcription
59406	1	335924	5	NULL	NULL	0	NULL	apoptosis			is mediated by					ceramide					NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_152	9415703	Ceramide-mediated apoptosis was unaffected by the ceramide acylhydrolase inhibitor oleoylethanolamine (Table  3), indicating that deacylation to sphingosine did not underlie the bioactivity of ceramide.	transcription
59407	2	335924	5	NULL	NULL	0	NULL	oleoylethanolamine			does not affect					statement 1					NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_152	9415703	Ceramide-mediated apoptosis was unaffected by the ceramide acylhydrolase inhibitor oleoylethanolamine (Table  3), indicating that deacylation to sphingosine did not underlie the bioactivity of ceramide.	transcription
59408	3	335924	5	NULL	NULL	0	NULL	oleoylethanolamine			is an inhibitor of					ceramide acylhydrolase					NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_152	9415703	Ceramide-mediated apoptosis was unaffected by the ceramide acylhydrolase inhibitor oleoylethanolamine (Table  3), indicating that deacylation to sphingosine did not underlie the bioactivity of ceramide.	transcription
59409	4	335924	5	NULL	NULL	0	NULL	sphingosine		deacylation to	does not underlie					ceramide		bioactivity of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_152	9415703	Ceramide-mediated apoptosis was unaffected by the ceramide acylhydrolase inhibitor oleoylethanolamine (Table  3), indicating that deacylation to sphingosine did not underlie the bioactivity of ceramide.	transcription
59410	5	335924	5	NULL	NULL	0	NULL	statement 3			indicates					statement 4					NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_152	9415703	Ceramide-mediated apoptosis was unaffected by the ceramide acylhydrolase inhibitor oleoylethanolamine (Table  3), indicating that deacylation to sphingosine did not underlie the bioactivity of ceramide.	transcription
79366	1	335924	6	NULL	NULL	0	NULL	ceramide	Chemical		mediates					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_152	9415703	Ceramide-mediated apoptosis was unaffected by the ceramide acylhydrolase inhibitor oleoylethanolamine (Table  3), indicating that deacylation to sphingosine did not underlie the bioactivity of ceramide.	transcription
79367	2	335924	6	NULL	NULL	0	NULL	oleoylethanolamine	Chemical		does not affect					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_152	9415703	Ceramide-mediated apoptosis was unaffected by the ceramide acylhydrolase inhibitor oleoylethanolamine (Table  3), indicating that deacylation to sphingosine did not underlie the bioactivity of ceramide.	transcription
79368	3	335924	6	NULL	NULL	0	NULL	oleoylethanolamine	Chemical		is a type of					ceramide acylhydrolase inhibitor	Chemical				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_152	9415703	Ceramide-mediated apoptosis was unaffected by the ceramide acylhydrolase inhibitor oleoylethanolamine (Table  3), indicating that deacylation to sphingosine did not underlie the bioactivity of ceramide.	transcription
59411	1	335925	5	NULL	NULL	0	NULL	phospholipase D			is activated by					sphingosine 1-phosphate					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_7	7592842	C - and  C -ceramides blocked the activation of phospholipase D by  sphingosine 1-phosphate, and this inhibition was not affected by  insulin.	transcription
59412	2	335925	5	NULL	NULL	0	NULL	C -ceramides			blocks					statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_7	7592842	C - and  C -ceramides blocked the activation of phospholipase D by  sphingosine 1-phosphate, and this inhibition was not affected by  insulin.	transcription
59413	3	335925	5	NULL	NULL	0	NULL	insulin			does not affect					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_7	7592842	C - and  C -ceramides blocked the activation of phospholipase D by  sphingosine 1-phosphate, and this inhibition was not affected by  insulin.	transcription
79363	1	335925	6	NULL	NULL	0	NULL	C-ceramides	Chemical		blocks					phospholipase D	GP	activation of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_7	7592842	C - and  C -ceramides blocked the activation of phospholipase D by  sphingosine 1-phosphate, and this inhibition was not affected by  insulin.	transcription
79364	2	335925	6	NULL	NULL	0	NULL	sphingosine 1-phosphate	GP		blocks					phospholipase D	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_7	7592842	C - and  C -ceramides blocked the activation of phospholipase D by  sphingosine 1-phosphate, and this inhibition was not affected by  insulin.	transcription
79365	3	335925	6	NULL	NULL	0	NULL	Insulin	GP		does not affect					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_7	7592842	C - and  C -ceramides blocked the activation of phospholipase D by  sphingosine 1-phosphate, and this inhibition was not affected by  insulin.	transcription
59414	1	335926	5	NULL	NULL	0	NULL	C6-ceramide			is					N-hexanoyl sphingosine					NULL		0	NULL	NULL	NULL	abs-batch0600-0619_j-biochem-(tokyo)_139_2_16452313_s_5	16452313	We found that N-hexanoyl sphingosine (C6-ceramide)  induced apoptosis efficiently through the accumulation of long chain ceramides.	transcription
59415	2	335926	5	NULL	NULL	0	NULL	C6-ceramide			induce		efficiently			apoptosis					NULL		0	NULL	NULL	NULL	abs-batch0600-0619_j-biochem-(tokyo)_139_2_16452313_s_5	16452313	We found that N-hexanoyl sphingosine (C6-ceramide)  induced apoptosis efficiently through the accumulation of long chain ceramides.	transcription
59416	3	335926	5	NULL	NULL	0	NULL	statement 2			occurs through					long chain ceramides		accumulation of			NULL		NULL	NULL	NULL	NULL	abs-batch0600-0619_j-biochem-(tokyo)_139_2_16452313_s_5	16452313	We found that N-hexanoyl sphingosine (C6-ceramide)  induced apoptosis efficiently through the accumulation of long chain ceramides.	transcription
79361	1	335926	6	NULL	NULL	0	NULL	N-hexanoyl sphingosine	Chemical		induces					apoptosis	Process				NULL		0	NULL	NULL	NULL	abs-batch0600-0619_j-biochem-(tokyo)_139_2_16452313_s_5	16452313	We found that N-hexanoyl sphingosine (C6-ceramide)  induced apoptosis efficiently through the accumulation of long chain ceramides.	transcription
79362	2	335926	6	NULL	NULL	0	NULL	N-hexanoyl sphingosine	Chemical		is					C6-ceramide	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0600-0619_j-biochem-(tokyo)_139_2_16452313_s_5	16452313	We found that N-hexanoyl sphingosine (C6-ceramide)  induced apoptosis efficiently through the accumulation of long chain ceramides.	transcription
59417	1	335927	5	NULL	NULL	0	NULL	C2-ceramide			is					N-acetyl sphingosine					NULL		0	NULL	NULL	NULL	abs-batch0600-0619_j-biochem-(tokyo)_139_2_16452313_s_6	16452313	On the other hand, N-acetyl sphingosine (C2-ceramide) induced neither  apoptosis nor accumulation of long chain ceramides.	transcription
59418	2	335927	5	NULL	NULL	0	NULL	C2-ceramide			does not induce					apoptosis					NULL		0	NULL	NULL	NULL	abs-batch0600-0619_j-biochem-(tokyo)_139_2_16452313_s_6	16452313	On the other hand, N-acetyl sphingosine (C2-ceramide) induced neither  apoptosis nor accumulation of long chain ceramides.	transcription
59419	3	335927	5	NULL	NULL	0	NULL	C2-ceramide			does not induce					long chain ceramides		accumulation of			NULL		0	NULL	NULL	NULL	abs-batch0600-0619_j-biochem-(tokyo)_139_2_16452313_s_6	16452313	On the other hand, N-acetyl sphingosine (C2-ceramide) induced neither  apoptosis nor accumulation of long chain ceramides.	transcription
79359	1	335927	6	NULL	NULL	0	NULL	N-acetyl sphingosine	Chemical		does not induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	abs-batch0600-0619_j-biochem-(tokyo)_139_2_16452313_s_6	16452313	On the other hand, N-acetyl sphingosine (C2-ceramide) induced neither  apoptosis nor accumulation of long chain ceramides.	transcription
79360	2	335927	6	NULL	NULL	0	NULL	N-acetyl sphingosine	Chemical		does not induce					ceramide	Chemical	accumulation of;; long chain			NULL		0	NULL	NULL	NULL	abs-batch0600-0619_j-biochem-(tokyo)_139_2_16452313_s_6	16452313	On the other hand, N-acetyl sphingosine (C2-ceramide) induced neither  apoptosis nor accumulation of long chain ceramides.	transcription
59420	1	335928	5	NULL	NULL	0	NULL	haCER2			is					human ceramidase					NULL		0	NULL	NULL	NULL	abs-batch0760-0779_faseb-j_20_11_16940153_s_4	16940153	Here we identify a novel human ceramidase (haCER2) that regulates the  levels of both sphingosine and S1P by controlling the hydrolysis of ceramides.	transcription
59421	2	335928	5	NULL	NULL	0	NULL	haCER2			regulates					sphingosine		level of			NULL		NULL	NULL	NULL	NULL	abs-batch0760-0779_faseb-j_20_11_16940153_s_4	16940153	Here we identify a novel human ceramidase (haCER2) that regulates the  levels of both sphingosine and S1P by controlling the hydrolysis of ceramides.	transcription
59422	3	335928	5	NULL	NULL	0	NULL	haCER2			controls					ceramide		hydrolysis of			NULL		0	NULL	NULL	NULL	abs-batch0760-0779_faseb-j_20_11_16940153_s_4	16940153	Here we identify a novel human ceramidase (haCER2) that regulates the  levels of both sphingosine and S1P by controlling the hydrolysis of ceramides.	transcription
59423	4	335928	5	NULL	NULL	0	NULL	statement 3			leads to					statement 2					NULL		0	NULL	NULL	NULL	abs-batch0760-0779_faseb-j_20_11_16940153_s_4	16940153	Here we identify a novel human ceramidase (haCER2) that regulates the  levels of both sphingosine and S1P by controlling the hydrolysis of ceramides.	transcription
59424	5	335928	5	NULL	NULL	0	NULL	haCER2			regulates					S1P		level of			NULL		0	NULL	NULL	NULL	abs-batch0760-0779_faseb-j_20_11_16940153_s_4	16940153	Here we identify a novel human ceramidase (haCER2) that regulates the  levels of both sphingosine and S1P by controlling the hydrolysis of ceramides.	transcription
59425	6	335928	5	NULL	NULL	0	NULL	statement 3			leads to					statement 5					NULL		0	NULL	NULL	NULL	abs-batch0760-0779_faseb-j_20_11_16940153_s_4	16940153	Here we identify a novel human ceramidase (haCER2) that regulates the  levels of both sphingosine and S1P by controlling the hydrolysis of ceramides.	transcription
79355	1	335928	6	NULL	NULL	NULL	NULL	haCER2	GP		controls					ceramide	Chemical	hydrolysis of 			NULL		NULL	NULL	NULL	NULL	abs-batch0760-0779_faseb-j_20_11_16940153_s_4	16940153	Here we identify a novel human ceramidase (haCER2) that regulates the  levels of both sphingosine and S1P by controlling the hydrolysis of ceramides.	transcription
79356	2	335928	6	NULL	NULL	0	NULL	haCER2	GP		regulates					sphingosine	Chemical	levels of 			NULL		0	NULL	NULL	NULL	abs-batch0760-0779_faseb-j_20_11_16940153_s_4	16940153	Here we identify a novel human ceramidase (haCER2) that regulates the  levels of both sphingosine and S1P by controlling the hydrolysis of ceramides.	transcription
79357	3	335928	6	NULL	NULL	0	NULL	haCER2	GP		regulates					S1P	GP	levels of 			NULL		0	NULL	NULL	NULL	abs-batch0760-0779_faseb-j_20_11_16940153_s_4	16940153	Here we identify a novel human ceramidase (haCER2) that regulates the  levels of both sphingosine and S1P by controlling the hydrolysis of ceramides.	transcription
79358	4	335928	6	NULL	NULL	0	NULL	haCER2	GP		is					human ceramidase	GP				NULL		0	NULL	NULL	NULL	abs-batch0760-0779_faseb-j_20_11_16940153_s_4	16940153	Here we identify a novel human ceramidase (haCER2) that regulates the  levels of both sphingosine and S1P by controlling the hydrolysis of ceramides.	transcription
59426	1	335929	5	NULL	NULL	0	NULL	ceramide			induce					apoptosis					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_30_19060_s_144	9668088	Although PAP1 might also be toxic as a ceramide analog because ceramides can induce apoptosis, this probably does not play a role in the toxicity of PAP1 because the effects of N-acylsphingosines (ceramides) are usually stereoselective and require the 4,5- trans-double bond of the sphingosine backbone ( 28).	transcription
59427	2	335929	5	NULL	NULL	0	NULL	sphingosine			does not play a role in					PAP1		toxicity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_30_19060_s_144	9668088	Although PAP1 might also be toxic as a ceramide analog because ceramides can induce apoptosis, this probably does not play a role in the toxicity of PAP1 because the effects of N-acylsphingosines (ceramides) are usually stereoselective and require the 4,5- trans-double bond of the sphingosine backbone ( 28).	transcription
59428	1	335930	5	NULL	NULL	0	NULL	serum		deprivation of	is an inducer of					stress					NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_156	12531549	Accordingly, enforced expression of sphingosine kinase markedly enhanced survival in NIH3T3 [  90], HEK293 [ 90], Jurkat [ 90], and PC12 cells [ 88] in response to several stress inducers such as serum deprivation, Fas ligation, bacterial sphingomyelinase, and cell-permeable ceramides known to increase cellular ceramide and sphingosine levels.	transcription
59429	2	335930	5	NULL	NULL	0	NULL	Fas		ligation of	is an inducer of					stress					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_156	12531549	Accordingly, enforced expression of sphingosine kinase markedly enhanced survival in NIH3T3 [  90], HEK293 [ 90], Jurkat [ 90], and PC12 cells [ 88] in response to several stress inducers such as serum deprivation, Fas ligation, bacterial sphingomyelinase, and cell-permeable ceramides known to increase cellular ceramide and sphingosine levels.	transcription
59430	3	335930	5	NULL	NULL	0	NULL	sphingomyelinase		bacterial	is an inducer of					stress					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_156	12531549	Accordingly, enforced expression of sphingosine kinase markedly enhanced survival in NIH3T3 [  90], HEK293 [ 90], Jurkat [ 90], and PC12 cells [ 88] in response to several stress inducers such as serum deprivation, Fas ligation, bacterial sphingomyelinase, and cell-permeable ceramides known to increase cellular ceramide and sphingosine levels.	transcription
59431	4	335930	5	NULL	NULL	0	NULL	ceramide		cell-permeable	is an inducer of					stress					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_156	12531549	Accordingly, enforced expression of sphingosine kinase markedly enhanced survival in NIH3T3 [  90], HEK293 [ 90], Jurkat [ 90], and PC12 cells [ 88] in response to several stress inducers such as serum deprivation, Fas ligation, bacterial sphingomyelinase, and cell-permeable ceramides known to increase cellular ceramide and sphingosine levels.	transcription
59432	5	335930	5	NULL	NULL	0	NULL	serum		deprivation of	increases					ceramide		cellular levels of			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_156	12531549	Accordingly, enforced expression of sphingosine kinase markedly enhanced survival in NIH3T3 [  90], HEK293 [ 90], Jurkat [ 90], and PC12 cells [ 88] in response to several stress inducers such as serum deprivation, Fas ligation, bacterial sphingomyelinase, and cell-permeable ceramides known to increase cellular ceramide and sphingosine levels.	transcription
59433	6	335930	5	NULL	NULL	0	NULL	Fas		ligation of	increases					ceramide		cellular levels of			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_156	12531549	Accordingly, enforced expression of sphingosine kinase markedly enhanced survival in NIH3T3 [  90], HEK293 [ 90], Jurkat [ 90], and PC12 cells [ 88] in response to several stress inducers such as serum deprivation, Fas ligation, bacterial sphingomyelinase, and cell-permeable ceramides known to increase cellular ceramide and sphingosine levels.	transcription
59434	7	335930	5	NULL	NULL	0	NULL	sphingomyelinase		bacterial	increases					ceramide		cellular levels of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_156	12531549	Accordingly, enforced expression of sphingosine kinase markedly enhanced survival in NIH3T3 [  90], HEK293 [ 90], Jurkat [ 90], and PC12 cells [ 88] in response to several stress inducers such as serum deprivation, Fas ligation, bacterial sphingomyelinase, and cell-permeable ceramides known to increase cellular ceramide and sphingosine levels.	transcription
59435	8	335930	5	NULL	NULL	0	NULL	ceramide		cell-permeable	increases					ceramide		cellular levels of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_156	12531549	Accordingly, enforced expression of sphingosine kinase markedly enhanced survival in NIH3T3 [  90], HEK293 [ 90], Jurkat [ 90], and PC12 cells [ 88] in response to several stress inducers such as serum deprivation, Fas ligation, bacterial sphingomyelinase, and cell-permeable ceramides known to increase cellular ceramide and sphingosine levels.	transcription
59436	9	335930	5	NULL	NULL	0	NULL	serum		deprivation of	increases					sphingosine		cellular levels of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_156	12531549	Accordingly, enforced expression of sphingosine kinase markedly enhanced survival in NIH3T3 [  90], HEK293 [ 90], Jurkat [ 90], and PC12 cells [ 88] in response to several stress inducers such as serum deprivation, Fas ligation, bacterial sphingomyelinase, and cell-permeable ceramides known to increase cellular ceramide and sphingosine levels.	transcription
59437	10	335930	5	NULL	NULL	0	NULL	Fas`		ligation of	increases					sphingosine		cellular levels of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_156	12531549	Accordingly, enforced expression of sphingosine kinase markedly enhanced survival in NIH3T3 [  90], HEK293 [ 90], Jurkat [ 90], and PC12 cells [ 88] in response to several stress inducers such as serum deprivation, Fas ligation, bacterial sphingomyelinase, and cell-permeable ceramides known to increase cellular ceramide and sphingosine levels.	transcription
59438	11	335930	5	NULL	NULL	0	NULL	sphingomyelinase		bacterial	increases					sphingosine		cellular levels of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_156	12531549	Accordingly, enforced expression of sphingosine kinase markedly enhanced survival in NIH3T3 [  90], HEK293 [ 90], Jurkat [ 90], and PC12 cells [ 88] in response to several stress inducers such as serum deprivation, Fas ligation, bacterial sphingomyelinase, and cell-permeable ceramides known to increase cellular ceramide and sphingosine levels.	transcription
59439	12	335930	5	NULL	NULL	0	NULL	ceramide		cell-permeable	increases					sphingosine		cellular levels of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_156	12531549	Accordingly, enforced expression of sphingosine kinase markedly enhanced survival in NIH3T3 [  90], HEK293 [ 90], Jurkat [ 90], and PC12 cells [ 88] in response to several stress inducers such as serum deprivation, Fas ligation, bacterial sphingomyelinase, and cell-permeable ceramides known to increase cellular ceramide and sphingosine levels.	transcription
79347	1	335930	6	NULL	NULL	0	NULL	serum	GP	deprivation of 	induces					ceramide	Chemical	levels of 			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_156	12531549	Accordingly, enforced expression of sphingosine kinase markedly enhanced survival in NIH3T3 [  90], HEK293 [ 90], Jurkat [ 90], and PC12 cells [ 88] in response to several stress inducers such as serum deprivation, Fas ligation, bacterial sphingomyelinase, and cell-permeable ceramides known to increase cellular ceramide and sphingosine levels.	transcription
79348	2	335930	6	NULL	NULL	0	NULL	Fas	GP	ligation of 	induces					ceramide	Chemical	levels of 			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_156	12531549	Accordingly, enforced expression of sphingosine kinase markedly enhanced survival in NIH3T3 [  90], HEK293 [ 90], Jurkat [ 90], and PC12 cells [ 88] in response to several stress inducers such as serum deprivation, Fas ligation, bacterial sphingomyelinase, and cell-permeable ceramides known to increase cellular ceramide and sphingosine levels.	transcription
79349	3	335930	6	NULL	NULL	0	NULL	sphingomyelinase	GP	bacterial	induces					ceramide	Chemical	levels of 			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_156	12531549	Accordingly, enforced expression of sphingosine kinase markedly enhanced survival in NIH3T3 [  90], HEK293 [ 90], Jurkat [ 90], and PC12 cells [ 88] in response to several stress inducers such as serum deprivation, Fas ligation, bacterial sphingomyelinase, and cell-permeable ceramides known to increase cellular ceramide and sphingosine levels.	transcription
79350	4	335930	6	NULL	NULL	0	NULL	cell-permeable ceramides	Chemical		induces					ceramide	Chemical	levels of 			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_156	12531549	Accordingly, enforced expression of sphingosine kinase markedly enhanced survival in NIH3T3 [  90], HEK293 [ 90], Jurkat [ 90], and PC12 cells [ 88] in response to several stress inducers such as serum deprivation, Fas ligation, bacterial sphingomyelinase, and cell-permeable ceramides known to increase cellular ceramide and sphingosine levels.	transcription
79351	5	335930	6	NULL	NULL	0	NULL	serum	Chemical	deprivation of 	induces					sphingosine	Chemical	levels of 			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_156	12531549	Accordingly, enforced expression of sphingosine kinase markedly enhanced survival in NIH3T3 [  90], HEK293 [ 90], Jurkat [ 90], and PC12 cells [ 88] in response to several stress inducers such as serum deprivation, Fas ligation, bacterial sphingomyelinase, and cell-permeable ceramides known to increase cellular ceramide and sphingosine levels.	transcription
79352	6	335930	6	NULL	NULL	0	NULL	Fas	GP	ligation of 	induces					sphingosine	Chemical	levels of 			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_156	12531549	Accordingly, enforced expression of sphingosine kinase markedly enhanced survival in NIH3T3 [  90], HEK293 [ 90], Jurkat [ 90], and PC12 cells [ 88] in response to several stress inducers such as serum deprivation, Fas ligation, bacterial sphingomyelinase, and cell-permeable ceramides known to increase cellular ceramide and sphingosine levels.	transcription
79353	7	335930	6	NULL	NULL	0	NULL	sphingomyelinase	GP		increases					sphingosine	Chemical	levels of 			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_156	12531549	Accordingly, enforced expression of sphingosine kinase markedly enhanced survival in NIH3T3 [  90], HEK293 [ 90], Jurkat [ 90], and PC12 cells [ 88] in response to several stress inducers such as serum deprivation, Fas ligation, bacterial sphingomyelinase, and cell-permeable ceramides known to increase cellular ceramide and sphingosine levels.	transcription
79354	8	335930	6	NULL	NULL	0	NULL	cell-permeable ceramides	Chemical		increases					sphingosine	Chemical	levels of 			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_156	12531549	Accordingly, enforced expression of sphingosine kinase markedly enhanced survival in NIH3T3 [  90], HEK293 [ 90], Jurkat [ 90], and PC12 cells [ 88] in response to several stress inducers such as serum deprivation, Fas ligation, bacterial sphingomyelinase, and cell-permeable ceramides known to increase cellular ceramide and sphingosine levels.	transcription
59440	1	335932	5	NULL	NULL	0	NULL	palmitate			is incorporated into					ceramide					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_44_37118_s_312	16118219	Importantly, sphingosine-induced incorporation of [3]palmitate into ceramide ( Fig. 11 D) and sphingosine-induced increases in the major ceramide species were sharply curtailed by down-regulation of SphK2 ( Fig. 11 F), further suggesting a role for SphK2 in reutilization of sphingosine and its conversion to ceramide.	transcription
59441	2	335932	5	NULL	NULL	0	NULL	sphingosine			induce					statement 1					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_44_37118_s_312	16118219	Importantly, sphingosine-induced incorporation of [3]palmitate into ceramide ( Fig. 11 D) and sphingosine-induced increases in the major ceramide species were sharply curtailed by down-regulation of SphK2 ( Fig. 11 F), further suggesting a role for SphK2 in reutilization of sphingosine and its conversion to ceramide.	transcription
59442	3	335932	5	NULL	NULL	0	NULL	sphingosine			induce					ceramide species		increase in			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_44_37118_s_312	16118219	Importantly, sphingosine-induced incorporation of [3]palmitate into ceramide ( Fig. 11 D) and sphingosine-induced increases in the major ceramide species were sharply curtailed by down-regulation of SphK2 ( Fig. 11 F), further suggesting a role for SphK2 in reutilization of sphingosine and its conversion to ceramide.	transcription
59443	4	335932	5	NULL	NULL	0	NULL	SphK2		down-regulation of	curtails		sharply			statement 2					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_44_37118_s_312	16118219	Importantly, sphingosine-induced incorporation of [3]palmitate into ceramide ( Fig. 11 D) and sphingosine-induced increases in the major ceramide species were sharply curtailed by down-regulation of SphK2 ( Fig. 11 F), further suggesting a role for SphK2 in reutilization of sphingosine and its conversion to ceramide.	transcription
59444	5	335932	5	NULL	NULL	0	NULL	SphK2		down-regulation of	curtails		sharply			statement 3					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_44_37118_s_312	16118219	Importantly, sphingosine-induced incorporation of [3]palmitate into ceramide ( Fig. 11 D) and sphingosine-induced increases in the major ceramide species were sharply curtailed by down-regulation of SphK2 ( Fig. 11 F), further suggesting a role for SphK2 in reutilization of sphingosine and its conversion to ceramide.	transcription
59445	6	335932	5	NULL	NULL	0	NULL	SphK2			plays a role in		may			sphingosine		reutilization of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_44_37118_s_312	16118219	Importantly, sphingosine-induced incorporation of [3]palmitate into ceramide ( Fig. 11 D) and sphingosine-induced increases in the major ceramide species were sharply curtailed by down-regulation of SphK2 ( Fig. 11 F), further suggesting a role for SphK2 in reutilization of sphingosine and its conversion to ceramide.	transcription
59446	7	335932	5	NULL	NULL	0	NULL	sphingosine			is converted to					ceramide					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_44_37118_s_312	16118219	Importantly, sphingosine-induced incorporation of [3]palmitate into ceramide ( Fig. 11 D) and sphingosine-induced increases in the major ceramide species were sharply curtailed by down-regulation of SphK2 ( Fig. 11 F), further suggesting a role for SphK2 in reutilization of sphingosine and its conversion to ceramide.	transcription
59447	8	335932	5	NULL	NULL	0	NULL	SphK2		down-regulation of	plays a role in		may			statement 7					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_44_37118_s_312	16118219	Importantly, sphingosine-induced incorporation of [3]palmitate into ceramide ( Fig. 11 D) and sphingosine-induced increases in the major ceramide species were sharply curtailed by down-regulation of SphK2 ( Fig. 11 F), further suggesting a role for SphK2 in reutilization of sphingosine and its conversion to ceramide.	transcription
79342	1	335932	6	NULL	NULL	0	NULL	palmitate	Chemical		is converted to					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_44_37118_s_312	16118219	Importantly, sphingosine-induced incorporation of [3]palmitate into ceramide ( Fig. 11 D) and sphingosine-induced increases in the major ceramide species were sharply curtailed by down-regulation of SphK2 ( Fig. 11 F), further suggesting a role for SphK2 in reutilization of sphingosine and its conversion to ceramide.	transcription
79343	2	335932	6	NULL	NULL	0	NULL	sphingosine	Chemical		induces					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_44_37118_s_312	16118219	Importantly, sphingosine-induced incorporation of [3]palmitate into ceramide ( Fig. 11 D) and sphingosine-induced increases in the major ceramide species were sharply curtailed by down-regulation of SphK2 ( Fig. 11 F), further suggesting a role for SphK2 in reutilization of sphingosine and its conversion to ceramide.	transcription
79344	3	335932	6	NULL	NULL	0	NULL	SphK2	GP		plays a role in					sphingosine	Chemical	reutilization of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_44_37118_s_312	16118219	Importantly, sphingosine-induced incorporation of [3]palmitate into ceramide ( Fig. 11 D) and sphingosine-induced increases in the major ceramide species were sharply curtailed by down-regulation of SphK2 ( Fig. 11 F), further suggesting a role for SphK2 in reutilization of sphingosine and its conversion to ceramide.	transcription
79345	4	335932	6	NULL	NULL	0	NULL	sphingosine	Chemical		is converted to					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_44_37118_s_312	16118219	Importantly, sphingosine-induced incorporation of [3]palmitate into ceramide ( Fig. 11 D) and sphingosine-induced increases in the major ceramide species were sharply curtailed by down-regulation of SphK2 ( Fig. 11 F), further suggesting a role for SphK2 in reutilization of sphingosine and its conversion to ceramide.	transcription
79346	5	335932	6	NULL	NULL	0	NULL	SphK2	GP		plays a role in					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_44_37118_s_312	16118219	Importantly, sphingosine-induced incorporation of [3]palmitate into ceramide ( Fig. 11 D) and sphingosine-induced increases in the major ceramide species were sharply curtailed by down-regulation of SphK2 ( Fig. 11 F), further suggesting a role for SphK2 in reutilization of sphingosine and its conversion to ceramide.	transcription
59448	1	335933	5	NULL	NULL	0	NULL	ceramide			is a type of					metabolite					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_57	12531549	Ceramide and sphingosine are interconvertible metabolites; however, sphingosine induces apoptosis without being converted to ceramide inasmuch as the ceramide synthase inhibitor fumonisin B1 does not affect sphingosine-induced apoptosis in HL-60 [  20,   21 and   22], U937 [  23], Jurkat [ 6, TF1 erythroleukemic [  24], and Hep3B hepatoma cells [  25].	transcription
59449	1	335933	5	NULL	NULL	0	NULL	ceramide			is a type of					metabolite					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_57	12531549	Ceramide and sphingosine are interconvertible metabolites; however, sphingosine induces apoptosis without being converted to ceramide inasmuch as the ceramide synthase inhibitor fumonisin B1 does not affect sphingosine-induced apoptosis in HL-60 [  20,   21 and   22], U937 [  23], Jurkat [ 6, TF1 erythroleukemic [  24], and Hep3B hepatoma cells [  25].	transcription
59450	2	335933	5	NULL	NULL	0	NULL	sphingosine			is a type of					metabolite					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_57	12531549	Ceramide and sphingosine are interconvertible metabolites; however, sphingosine induces apoptosis without being converted to ceramide inasmuch as the ceramide synthase inhibitor fumonisin B1 does not affect sphingosine-induced apoptosis in HL-60 [  20,   21 and   22], U937 [  23], Jurkat [ 6, TF1 erythroleukemic [  24], and Hep3B hepatoma cells [  25].	transcription
59451	3	335933	5	NULL	NULL	0	NULL	ceramide			is interconvertible to					sphingosine					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_57	12531549	Ceramide and sphingosine are interconvertible metabolites; however, sphingosine induces apoptosis without being converted to ceramide inasmuch as the ceramide synthase inhibitor fumonisin B1 does not affect sphingosine-induced apoptosis in HL-60 [  20,   21 and   22], U937 [  23], Jurkat [ 6, TF1 erythroleukemic [  24], and Hep3B hepatoma cells [  25].	transcription
59452	4	335933	5	NULL	NULL	0	NULL	sphingosine			induce					apoptosis					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_57	12531549	Ceramide and sphingosine are interconvertible metabolites; however, sphingosine induces apoptosis without being converted to ceramide inasmuch as the ceramide synthase inhibitor fumonisin B1 does not affect sphingosine-induced apoptosis in HL-60 [  20,   21 and   22], U937 [  23], Jurkat [ 6, TF1 erythroleukemic [  24], and Hep3B hepatoma cells [  25].	transcription
59453	5	335933	5	NULL	NULL	0	NULL	sphingosine			is not converted to					ceramide					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_57	12531549	Ceramide and sphingosine are interconvertible metabolites; however, sphingosine induces apoptosis without being converted to ceramide inasmuch as the ceramide synthase inhibitor fumonisin B1 does not affect sphingosine-induced apoptosis in HL-60 [  20,   21 and   22], U937 [  23], Jurkat [ 6, TF1 erythroleukemic [  24], and Hep3B hepatoma cells [  25].	transcription
59454	6	335933	5	NULL	NULL	0	NULL	statement 5			is necessary for					statement 4					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_57	12531549	Ceramide and sphingosine are interconvertible metabolites; however, sphingosine induces apoptosis without being converted to ceramide inasmuch as the ceramide synthase inhibitor fumonisin B1 does not affect sphingosine-induced apoptosis in HL-60 [  20,   21 and   22], U937 [  23], Jurkat [ 6, TF1 erythroleukemic [  24], and Hep3B hepatoma cells [  25].	transcription
59455	7	335933	5	NULL	NULL	0	NULL	fumonisin B1			is an inhibitor of					ceramide synthase					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_57	12531549	Ceramide and sphingosine are interconvertible metabolites; however, sphingosine induces apoptosis without being converted to ceramide inasmuch as the ceramide synthase inhibitor fumonisin B1 does not affect sphingosine-induced apoptosis in HL-60 [  20,   21 and   22], U937 [  23], Jurkat [ 6, TF1 erythroleukemic [  24], and Hep3B hepatoma cells [  25].	transcription
59456	8	335933	5	NULL	NULL	0	NULL	fumonisin B1			does not affect					statement 4					NULL	HL-60 cells	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_57	12531549	Ceramide and sphingosine are interconvertible metabolites; however, sphingosine induces apoptosis without being converted to ceramide inasmuch as the ceramide synthase inhibitor fumonisin B1 does not affect sphingosine-induced apoptosis in HL-60 [  20,   21 and   22], U937 [  23], Jurkat [ 6, TF1 erythroleukemic [  24], and Hep3B hepatoma cells [  25].	transcription
59457	9	335933	5	NULL	NULL	0	NULL	fumonisin B1			does not affect					statement 4					NULL	U937 cells	0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_57	12531549	Ceramide and sphingosine are interconvertible metabolites; however, sphingosine induces apoptosis without being converted to ceramide inasmuch as the ceramide synthase inhibitor fumonisin B1 does not affect sphingosine-induced apoptosis in HL-60 [  20,   21 and   22], U937 [  23], Jurkat [ 6, TF1 erythroleukemic [  24], and Hep3B hepatoma cells [  25].	transcription
59458	10	335933	5	NULL	NULL	0	NULL	fumonisin B1			does not affect					statement 4					NULL	Jurkat cells	0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_57	12531549	Ceramide and sphingosine are interconvertible metabolites; however, sphingosine induces apoptosis without being converted to ceramide inasmuch as the ceramide synthase inhibitor fumonisin B1 does not affect sphingosine-induced apoptosis in HL-60 [  20,   21 and   22], U937 [  23], Jurkat [ 6, TF1 erythroleukemic [  24], and Hep3B hepatoma cells [  25].	transcription
59459	11	335933	5	NULL	NULL	0	NULL	fumonisin B1			does not affect					statement 4					NULL	Hep3B hepatoma cells	0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_57	12531549	Ceramide and sphingosine are interconvertible metabolites; however, sphingosine induces apoptosis without being converted to ceramide inasmuch as the ceramide synthase inhibitor fumonisin B1 does not affect sphingosine-induced apoptosis in HL-60 [  20,   21 and   22], U937 [  23], Jurkat [ 6, TF1 erythroleukemic [  24], and Hep3B hepatoma cells [  25].	transcription
79336	1	335933	6	NULL	NULL	0	NULL	sphingosine	Chemical		induces					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_57	12531549	Ceramide and sphingosine are interconvertible metabolites; however, sphingosine induces apoptosis without being converted to ceramide inasmuch as the ceramide synthase inhibitor fumonisin B1 does not affect sphingosine-induced apoptosis in HL-60 [  20,   21 and   22], U937 [  23], Jurkat [ 6, TF1 erythroleukemic [  24], and Hep3B hepatoma cells [  25].	transcription
79337	2	335933	6	NULL	NULL	NULL	NULL	fumonisin B1	Chemical		does not affect					statement 1	Process				NULL	HL-60 cells	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_57	12531549	Ceramide and sphingosine are interconvertible metabolites; however, sphingosine induces apoptosis without being converted to ceramide inasmuch as the ceramide synthase inhibitor fumonisin B1 does not affect sphingosine-induced apoptosis in HL-60 [  20,   21 and   22], U937 [  23], Jurkat [ 6, TF1 erythroleukemic [  24], and Hep3B hepatoma cells [  25].	transcription
79338	3	335933	6	NULL	NULL	NULL	NULL	fumonisin B1	Chemical		does not affect					statement 1	Process				NULL	U937 cells	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_57	12531549	Ceramide and sphingosine are interconvertible metabolites; however, sphingosine induces apoptosis without being converted to ceramide inasmuch as the ceramide synthase inhibitor fumonisin B1 does not affect sphingosine-induced apoptosis in HL-60 [  20,   21 and   22], U937 [  23], Jurkat [ 6, TF1 erythroleukemic [  24], and Hep3B hepatoma cells [  25].	transcription
79339	4	335933	6	NULL	NULL	NULL	NULL	fumonisin B1	Chemical		does not affect					statement 1	Process				NULL	Jurkat cells	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_57	12531549	Ceramide and sphingosine are interconvertible metabolites; however, sphingosine induces apoptosis without being converted to ceramide inasmuch as the ceramide synthase inhibitor fumonisin B1 does not affect sphingosine-induced apoptosis in HL-60 [  20,   21 and   22], U937 [  23], Jurkat [ 6, TF1 erythroleukemic [  24], and Hep3B hepatoma cells [  25].	transcription
79340	5	335933	6	NULL	NULL	0	NULL	fumonisin B1	Chemical		does not affect					statement 1	Process				NULL	TF1 erythroleukemic cells	0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_57	12531549	Ceramide and sphingosine are interconvertible metabolites; however, sphingosine induces apoptosis without being converted to ceramide inasmuch as the ceramide synthase inhibitor fumonisin B1 does not affect sphingosine-induced apoptosis in HL-60 [  20,   21 and   22], U937 [  23], Jurkat [ 6, TF1 erythroleukemic [  24], and Hep3B hepatoma cells [  25].	transcription
79341	6	335933	6	NULL	NULL	0	NULL	fumonisin B1	Chemical		does not affect					statement 1	Process				NULL	Hep3B hepatoma cells	0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_57	12531549	Ceramide and sphingosine are interconvertible metabolites; however, sphingosine induces apoptosis without being converted to ceramide inasmuch as the ceramide synthase inhibitor fumonisin B1 does not affect sphingosine-induced apoptosis in HL-60 [  20,   21 and   22], U937 [  23], Jurkat [ 6, TF1 erythroleukemic [  24], and Hep3B hepatoma cells [  25].	transcription
59460	1	335934	5	NULL	NULL	0	NULL	safingol			is an inhibitor of		competitive			sphingosine kinase					NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_44_9_1772_s_30	12777464	As a competitive inhibitor of sphingosine kinase ( ), safingol could prevent the formation of S1P from sphingosine, which in turn is exclusively formed from ceramide ( ).	transcription
59461	2	335934	5	NULL	NULL	0	NULL	S1P			is formed from					sphingosine					NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_9_1772_s_30	12777464	As a competitive inhibitor of sphingosine kinase ( ), safingol could prevent the formation of S1P from sphingosine, which in turn is exclusively formed from ceramide ( ).	transcription
59462	3	335934	5	NULL	NULL	0	NULL	safingol			prevents					statement 2					NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_9_1772_s_30	12777464	As a competitive inhibitor of sphingosine kinase ( ), safingol could prevent the formation of S1P from sphingosine, which in turn is exclusively formed from ceramide ( ).	transcription
59463	4	335934	5	NULL	NULL	0	NULL	sphingosine			is formed from		exclusively			ceramide					NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_9_1772_s_30	12777464	As a competitive inhibitor of sphingosine kinase ( ), safingol could prevent the formation of S1P from sphingosine, which in turn is exclusively formed from ceramide ( ).	transcription
79334	1	335934	6	NULL	NULL	0	NULL	sphingosine	Chemical		is formed from					S1P	GP				NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_9_1772_s_30	12777464	As a competitive inhibitor of sphingosine kinase ( ), safingol could prevent the formation of S1P from sphingosine, which in turn is exclusively formed from ceramide ( ).	transcription
79335	2	335934	6	NULL	NULL	0	NULL	safingol	Chemical		prevents					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_9_1772_s_30	12777464	As a competitive inhibitor of sphingosine kinase ( ), safingol could prevent the formation of S1P from sphingosine, which in turn is exclusively formed from ceramide ( ).	transcription
59464	1	335935	5	NULL	NULL	0	NULL	S1P			is a downstream metabolite of					ceramide					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_44_34628_s_25	10942778	In contrast, S1P, a downstream metabolite of ceramide, produced by phosphorylation of sphingosine following activation of sphingosine kinase, is mitogenic and regulates apoptosis in diverse cell types ( 12).	transcription
59465	2	335935	5	NULL	NULL	0	NULL	sphingosine			is phosphorylated to					S1P					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_44_34628_s_25	10942778	In contrast, S1P, a downstream metabolite of ceramide, produced by phosphorylation of sphingosine following activation of sphingosine kinase, is mitogenic and regulates apoptosis in diverse cell types ( 12).	transcription
59466	3	335935	5	NULL	NULL	0	NULL	sphingosine kinase			catalyzes					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_44_34628_s_25	10942778	In contrast, S1P, a downstream metabolite of ceramide, produced by phosphorylation of sphingosine following activation of sphingosine kinase, is mitogenic and regulates apoptosis in diverse cell types ( 12).	transcription
59467	4	335935	5	NULL	NULL	0	NULL	S1P			regulates					apoptosis					NULL	diverse cell types	0	NULL	NULL	NULL	gw60_jbiolchem_275_44_34628_s_25	10942778	In contrast, S1P, a downstream metabolite of ceramide, produced by phosphorylation of sphingosine following activation of sphingosine kinase, is mitogenic and regulates apoptosis in diverse cell types ( 12).	transcription
79330	1	335935	6	NULL	NULL	0	NULL	S1P	GP		produced by					sphingosine	Chemical	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_44_34628_s_25	10942778	In contrast, S1P, a downstream metabolite of ceramide, produced by phosphorylation of sphingosine following activation of sphingosine kinase, is mitogenic and regulates apoptosis in diverse cell types ( 12).	transcription
79331	2	335935	6	NULL	NULL	0	NULL	statement 1	Process		activates					sphingosine kinase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_44_34628_s_25	10942778	In contrast, S1P, a downstream metabolite of ceramide, produced by phosphorylation of sphingosine following activation of sphingosine kinase, is mitogenic and regulates apoptosis in diverse cell types ( 12).	transcription
79332	3	335935	6	NULL	NULL	0	NULL	S1P	GP		is					mitogenic	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_44_34628_s_25	10942778	In contrast, S1P, a downstream metabolite of ceramide, produced by phosphorylation of sphingosine following activation of sphingosine kinase, is mitogenic and regulates apoptosis in diverse cell types ( 12).	transcription
79333	4	335935	6	NULL	NULL	0	NULL	S1P	GP		regulates					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_44_34628_s_25	10942778	In contrast, S1P, a downstream metabolite of ceramide, produced by phosphorylation of sphingosine following activation of sphingosine kinase, is mitogenic and regulates apoptosis in diverse cell types ( 12).	transcription
59468	1	335936	5	NULL	NULL	0	NULL	ceramide			induce					apoptosis					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_10_6876_s_336	10702247	In addition cellular levels of sphingosine (the product of ceramidase) and sphingosine phosphate are critical for cellular well being in that they may mediate proliferation and oppose ceramide-induced apoptosis ( 41).	transcription
59469	2	335936	5	NULL	NULL	0	NULL	sphingosine		cellular levels of	oppose		may			statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_10_6876_s_336	10702247	In addition cellular levels of sphingosine (the product of ceramidase) and sphingosine phosphate are critical for cellular well being in that they may mediate proliferation and oppose ceramide-induced apoptosis ( 41).	transcription
59470	3	335936	5	NULL	NULL	0	NULL	sphingosine phosphate			oppose		may			statement 1					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_10_6876_s_336	10702247	In addition cellular levels of sphingosine (the product of ceramidase) and sphingosine phosphate are critical for cellular well being in that they may mediate proliferation and oppose ceramide-induced apoptosis ( 41).	transcription
59471	4	335936	5	NULL	NULL	0	NULL	sphingosine			is a product of					ceramidase					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_10_6876_s_336	10702247	In addition cellular levels of sphingosine (the product of ceramidase) and sphingosine phosphate are critical for cellular well being in that they may mediate proliferation and oppose ceramide-induced apoptosis ( 41).	transcription
79327	1	335936	6	NULL	NULL	0	NULL	sphingosine	Chemical		mediates					proliferation	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_10_6876_s_336	10702247	In addition cellular levels of sphingosine (the product of ceramidase) and sphingosine phosphate are critical for cellular well being in that they may mediate proliferation and oppose ceramide-induced apoptosis ( 41).	transcription
79328	2	335936	6	NULL	NULL	0	NULL	sphingosine phosphate	GP		mediates					proliferation	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_10_6876_s_336	10702247	In addition cellular levels of sphingosine (the product of ceramidase) and sphingosine phosphate are critical for cellular well being in that they may mediate proliferation and oppose ceramide-induced apoptosis ( 41).	transcription
79329	3	335936	6	NULL	NULL	0	NULL	ceramide	Chemical		induces					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_10_6876_s_336	10702247	In addition cellular levels of sphingosine (the product of ceramidase) and sphingosine phosphate are critical for cellular well being in that they may mediate proliferation and oppose ceramide-induced apoptosis ( 41).	transcription
59472	1	335937	5	NULL	NULL	0	NULL	ceramide		cell-permeable	does not stimulate					PLD					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_8_1244_s_346	12177168	Also, the cell-permeable [C2]ceramide, exogenous sphingomyelinase, or sphingosine failed to stimulate PLD, and sphingosine 1-phosphate was a weak activator of this enzyme activity in the acini.	transcription
59473	2	335937	5	NULL	NULL	0	NULL	sphingomyelinase		exogenous	does not stimulate					PLD					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_8_1244_s_346	12177168	Also, the cell-permeable [C2]ceramide, exogenous sphingomyelinase, or sphingosine failed to stimulate PLD, and sphingosine 1-phosphate was a weak activator of this enzyme activity in the acini.	transcription
59474	3	335937	5	NULL	NULL	0	NULL	sphingosine			does not stimulate					PLD					NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_8_1244_s_346	12177168	Also, the cell-permeable [C2]ceramide, exogenous sphingomyelinase, or sphingosine failed to stimulate PLD, and sphingosine 1-phosphate was a weak activator of this enzyme activity in the acini.	transcription
59475	4	335937	5	NULL	NULL	0	NULL	sphingosine 1-phosphate			activates		weakly			PLD		activity of			NULL	acini	0	NULL	NULL	NULL	gw60_jlipidres_43_8_1244_s_346	12177168	Also, the cell-permeable [C2]ceramide, exogenous sphingomyelinase, or sphingosine failed to stimulate PLD, and sphingosine 1-phosphate was a weak activator of this enzyme activity in the acini.	transcription
79324	1	335937	6	NULL	NULL	0	NULL	ceramide	Chemical		does not stimulate					PLD	GP				NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_8_1244_s_346	12177168	Also, the cell-permeable [C2]ceramide, exogenous sphingomyelinase, or sphingosine failed to stimulate PLD, and sphingosine 1-phosphate was a weak activator of this enzyme activity in the acini.	transcription
79325	2	335937	6	NULL	NULL	0	NULL	sphingosine	Chemical		does not stimulate					PLD	GP				NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_8_1244_s_346	12177168	Also, the cell-permeable [C2]ceramide, exogenous sphingomyelinase, or sphingosine failed to stimulate PLD, and sphingosine 1-phosphate was a weak activator of this enzyme activity in the acini.	transcription
79326	3	335937	6	NULL	NULL	0	NULL	sphingosine 1-phosphate	GP		does not stimulate					PLD	GP				NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_8_1244_s_346	12177168	Also, the cell-permeable [C2]ceramide, exogenous sphingomyelinase, or sphingosine failed to stimulate PLD, and sphingosine 1-phosphate was a weak activator of this enzyme activity in the acini.	transcription
59476	1	335938	5	NULL	NULL	0	NULL	ceramide	Chemical	cell-permeable	inhibit					sphingosine kinase-1	GP				NULL	chemoresistant cells	NULL	NULL	NULL	NULL	abs-batch0650-0679_leukemia_20_1_16281067_s_7	16281067	Incubation with cell-permeable ceramide of chemoresistant cells  led to a sphingosine kinase-1 inhibition and apoptosis both prevented  by sphingosine kinase-1 over-expression.	transcription
59477	2	335938	5	NULL	NULL	0	NULL	ceramide	Chemical	cell-permeable	leads to					apoptosis	Process				NULL	chemoresistant cells	0	NULL	NULL	NULL	abs-batch0650-0679_leukemia_20_1_16281067_s_7	16281067	Incubation with cell-permeable ceramide of chemoresistant cells  led to a sphingosine kinase-1 inhibition and apoptosis both prevented  by sphingosine kinase-1 over-expression.	transcription
59478	3	335938	5	NULL	NULL	0	NULL	statement 1	Process		prevented by					sphingosine kinase-1	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_leukemia_20_1_16281067_s_7	16281067	Incubation with cell-permeable ceramide of chemoresistant cells  led to a sphingosine kinase-1 inhibition and apoptosis both prevented  by sphingosine kinase-1 over-expression.	transcription
59479	4	335938	5	NULL	NULL	0	NULL	statement 2	Process		prevented by					sphingosine kinase-1	GP				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_leukemia_20_1_16281067_s_7	16281067	Incubation with cell-permeable ceramide of chemoresistant cells  led to a sphingosine kinase-1 inhibition and apoptosis both prevented  by sphingosine kinase-1 over-expression.	transcription
79320	1	335938	6	NULL	NULL	0	NULL	ceramide	Chemical		leads to					sphingosine kinase-1	GP	inhibition of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_leukemia_20_1_16281067_s_7	16281067	Incubation with cell-permeable ceramide of chemoresistant cells  led to a sphingosine kinase-1 inhibition and apoptosis both prevented  by sphingosine kinase-1 over-expression.	transcription
79321	2	335938	6	NULL	NULL	0	NULL	ceramide	Chemical		leads to					apoptosis	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_leukemia_20_1_16281067_s_7	16281067	Incubation with cell-permeable ceramide of chemoresistant cells  led to a sphingosine kinase-1 inhibition and apoptosis both prevented  by sphingosine kinase-1 over-expression.	transcription
79322	3	335938	6	NULL	NULL	0	NULL	sphingosine kinase-1	GP		prevents					statement 1	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_leukemia_20_1_16281067_s_7	16281067	Incubation with cell-permeable ceramide of chemoresistant cells  led to a sphingosine kinase-1 inhibition and apoptosis both prevented  by sphingosine kinase-1 over-expression.	transcription
79323	4	335938	6	NULL	NULL	0	NULL	sphingosine kinase-1	GP		prevents					statement 1	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_leukemia_20_1_16281067_s_7	16281067	Incubation with cell-permeable ceramide of chemoresistant cells  led to a sphingosine kinase-1 inhibition and apoptosis both prevented  by sphingosine kinase-1 over-expression.	transcription
59480	1	335939	5	NULL	NULL	0	NULL	TNF-alpha	GP		changes					ceramide	Chemical	levels of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_99_s_72	16269668	Cell transfection with N-SMase2 siRNA inhibited the changes induced by TNF-alpha in the levels not only of ceramide but also of sphingosine and Sph1P ( Figure 2A), whereas transfection with SK1-DN blocked generation of Sph1P with accumulation of sphingosine and ceramide ( Figure 2B).	transcription
59481	2	335939	5	NULL	NULL	0	NULL	TNF-alpha	GP		changes					sphingosine	Chemical	levels of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_99_s_72	16269668	Cell transfection with N-SMase2 siRNA inhibited the changes induced by TNF-alpha in the levels not only of ceramide but also of sphingosine and Sph1P ( Figure 2A), whereas transfection with SK1-DN blocked generation of Sph1P with accumulation of sphingosine and ceramide ( Figure 2B).	transcription
59482	3	335939	5	NULL	NULL	0	NULL	TNF-alpha	GP		changes					Sph1P	Chemical	levels of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_99_s_72	16269668	Cell transfection with N-SMase2 siRNA inhibited the changes induced by TNF-alpha in the levels not only of ceramide but also of sphingosine and Sph1P ( Figure 2A), whereas transfection with SK1-DN blocked generation of Sph1P with accumulation of sphingosine and ceramide ( Figure 2B).	transcription
59483	4	335939	5	NULL	NULL	0	NULL	N-SMase2 siRNA	NucleicAcid		inhibits					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_99_s_72	16269668	Cell transfection with N-SMase2 siRNA inhibited the changes induced by TNF-alpha in the levels not only of ceramide but also of sphingosine and Sph1P ( Figure 2A), whereas transfection with SK1-DN blocked generation of Sph1P with accumulation of sphingosine and ceramide ( Figure 2B).	transcription
59484	5	335939	5	NULL	NULL	0	NULL	N-SMase2 siRNA	NucleicAcid		inhibits					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_99_s_72	16269668	Cell transfection with N-SMase2 siRNA inhibited the changes induced by TNF-alpha in the levels not only of ceramide but also of sphingosine and Sph1P ( Figure 2A), whereas transfection with SK1-DN blocked generation of Sph1P with accumulation of sphingosine and ceramide ( Figure 2B).	transcription
59485	6	335939	5	NULL	NULL	0	NULL	N-SMase2 siRNA	NucleicAcid		inhibits					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_99_s_72	16269668	Cell transfection with N-SMase2 siRNA inhibited the changes induced by TNF-alpha in the levels not only of ceramide but also of sphingosine and Sph1P ( Figure 2A), whereas transfection with SK1-DN blocked generation of Sph1P with accumulation of sphingosine and ceramide ( Figure 2B).	transcription
59486	7	335939	5	NULL	NULL	0	NULL	SK1-DN	GP		block					Sph1P	Chemical	generation of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_99_s_72	16269668	Cell transfection with N-SMase2 siRNA inhibited the changes induced by TNF-alpha in the levels not only of ceramide but also of sphingosine and Sph1P ( Figure 2A), whereas transfection with SK1-DN blocked generation of Sph1P with accumulation of sphingosine and ceramide ( Figure 2B).	transcription
59487	8	335939	5	NULL	NULL	0	NULL	SK1-DN	GP		accumulates					sphingosine	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_99_s_72	16269668	Cell transfection with N-SMase2 siRNA inhibited the changes induced by TNF-alpha in the levels not only of ceramide but also of sphingosine and Sph1P ( Figure 2A), whereas transfection with SK1-DN blocked generation of Sph1P with accumulation of sphingosine and ceramide ( Figure 2B).	transcription
59488	9	335939	5	NULL	NULL	0	NULL	statement 8	Process		leads to					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_99_s_72	16269668	Cell transfection with N-SMase2 siRNA inhibited the changes induced by TNF-alpha in the levels not only of ceramide but also of sphingosine and Sph1P ( Figure 2A), whereas transfection with SK1-DN blocked generation of Sph1P with accumulation of sphingosine and ceramide ( Figure 2B).	transcription
59489	10	335939	5	NULL	NULL	0	NULL	SK1-DN	GP		accumulates					ceramide	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_99_s_72	16269668	Cell transfection with N-SMase2 siRNA inhibited the changes induced by TNF-alpha in the levels not only of ceramide but also of sphingosine and Sph1P ( Figure 2A), whereas transfection with SK1-DN blocked generation of Sph1P with accumulation of sphingosine and ceramide ( Figure 2B).	transcription
59490	11	335939	5	NULL	NULL	0	NULL	statement 10	Process		leads to					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_99_s_72	16269668	Cell transfection with N-SMase2 siRNA inhibited the changes induced by TNF-alpha in the levels not only of ceramide but also of sphingosine and Sph1P ( Figure 2A), whereas transfection with SK1-DN blocked generation of Sph1P with accumulation of sphingosine and ceramide ( Figure 2B).	transcription
59491	1	335940	5	NULL	NULL	0	NULL	ceramide	Chemical	increase in	more rapid than					sphingosine	Chemical	increase in			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_27	12531549	The increase in ceramide content was more rapid than that of sphingosine, suggesting that the increase of sphingosine levels could be resulting from the degradation of ceramide formed after TNF  treatment [ 5.	transcription
59492	2	335940	5	NULL	NULL	0	NULL	sphingosine	Chemical	increase in;;levels of	results from		may			ceramide	Chemical	degradation of			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_27	12531549	The increase in ceramide content was more rapid than that of sphingosine, suggesting that the increase of sphingosine levels could be resulting from the degradation of ceramide formed after TNF  treatment [ 5.	transcription
59493	3	335940	5	NULL	NULL	0	NULL	statement 2	Process		occurs after					TNF	GP	treatment			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_27	12531549	The increase in ceramide content was more rapid than that of sphingosine, suggesting that the increase of sphingosine levels could be resulting from the degradation of ceramide formed after TNF  treatment [ 5.	transcription
59494	4	335940	5	NULL	NULL	0	NULL	statement 1	Process		suggest					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_27	12531549	The increase in ceramide content was more rapid than that of sphingosine, suggesting that the increase of sphingosine levels could be resulting from the degradation of ceramide formed after TNF  treatment [ 5.	transcription
79318	1	335940	6	NULL	NULL	0	NULL	TNF	GP		degrades					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_27	12531549	The increase in ceramide content was more rapid than that of sphingosine, suggesting that the increase of sphingosine levels could be resulting from the degradation of ceramide formed after TNF  treatment [ 5.	transcription
79319	2	335940	6	NULL	NULL	0	NULL	statement 1	Process		increases					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_27	12531549	The increase in ceramide content was more rapid than that of sphingosine, suggesting that the increase of sphingosine levels could be resulting from the degradation of ceramide formed after TNF  treatment [ 5.	transcription
59495	1	335941	5	NULL	NULL	0	NULL	S1P	Chemical	dephosphorylation of;;exogenous	generates					sphingosine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_158_6_1039_s_94	12235122	Thus, it is most likely that as a consequence of overexpression of mSPP-1, the increased sphingosine generated by dephosphorylation of exogenous S1P has been diverted to ceramide generation by ceramide synthase - catalyzed N-acylation of sphingosine.	transcription
59496	3	335941	5	NULL	NULL	0	NULL	statement 2	Process		generates					ceramide	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_158_6_1039_s_94	12235122	Thus, it is most likely that as a consequence of overexpression of mSPP-1, the increased sphingosine generated by dephosphorylation of exogenous S1P has been diverted to ceramide generation by ceramide synthase - catalyzed N-acylation of sphingosine.	transcription
59497	2	335941	5	NULL	NULL	0	NULL	sphingosine	Chemical	N-acylation of	is catalyzed by					ceramide synthase	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_158_6_1039_s_94	12235122	Thus, it is most likely that as a consequence of overexpression of mSPP-1, the increased sphingosine generated by dephosphorylation of exogenous S1P has been diverted to ceramide generation by ceramide synthase - catalyzed N-acylation of sphingosine.	transcription
59498	4	335941	5	NULL	NULL	0	NULL	mSPP-1	GP	overexpression of	leads to					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_158_6_1039_s_94	12235122	Thus, it is most likely that as a consequence of overexpression of mSPP-1, the increased sphingosine generated by dephosphorylation of exogenous S1P has been diverted to ceramide generation by ceramide synthase - catalyzed N-acylation of sphingosine.	transcription
59499	1	335942	5	NULL	NULL	0	NULL	sphingosine	Chemical	addition of;;exogenous	elevates		rapidly			ceramide	Chemical	cellular levels of			NULL	A431 cells, Neuro2a cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_5_3028_s_253	9006952	Addition of exogenous sphingosine rapidly elevates cellular ceramide levels in A431 cells and Neuro2a cells ( 66,  67) suggesting that some effects of sphingosine may be mediated by its conversion to ceramide.	transcription
59500	2	335942	5	NULL	NULL	0	NULL	sphingosine	Chemical		is converted to					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_5_3028_s_253	9006952	Addition of exogenous sphingosine rapidly elevates cellular ceramide levels in A431 cells and Neuro2a cells ( 66,  67) suggesting that some effects of sphingosine may be mediated by its conversion to ceramide.	transcription
59501	3	335942	5	NULL	NULL	0	NULL	sphingosine	Chemical	effect of	is mediated by		may be			statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_5_3028_s_253	9006952	Addition of exogenous sphingosine rapidly elevates cellular ceramide levels in A431 cells and Neuro2a cells ( 66,  67) suggesting that some effects of sphingosine may be mediated by its conversion to ceramide.	transcription
79316	1	335942	6	NULL	NULL	0	NULL	sphingosine	Chemical		elevates					ceramide	Chemical				NULL	A431 cells	0	NULL	NULL	NULL	gw60_jbiolchem_272_5_3028_s_253	9006952	Addition of exogenous sphingosine rapidly elevates cellular ceramide levels in A431 cells and Neuro2a cells ( 66,  67) suggesting that some effects of sphingosine may be mediated by its conversion to ceramide.	transcription
79317	2	335942	6	NULL	NULL	0	NULL	sphingosine	Chemical		elevates					ceramide	Chemical	levels of 			NULL	Neuro2a cells	0	NULL	NULL	NULL	gw60_jbiolchem_272_5_3028_s_253	9006952	Addition of exogenous sphingosine rapidly elevates cellular ceramide levels in A431 cells and Neuro2a cells ( 66,  67) suggesting that some effects of sphingosine may be mediated by its conversion to ceramide.	transcription
59502	1	335943	5	NULL	NULL	0	NULL	PLD	GP		is activated by					ATP	Chemical				NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_8_1244_s_345	12177168	Our results indicate that it is unlikely that PLD activation by ATP is mediated by ceramide or its possible metabolism to sphingosine or sphingosine 1-phosphate, as ATP does not cause ceramide accumulation in the acini.	transcription
59503	2	335943	5	NULL	NULL	0	NULL	ceramide	Chemical		does not mediate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_43_8_1244_s_345	12177168	Our results indicate that it is unlikely that PLD activation by ATP is mediated by ceramide or its possible metabolism to sphingosine or sphingosine 1-phosphate, as ATP does not cause ceramide accumulation in the acini.	transcription
59504	3	335943	5	NULL	NULL	0	NULL	ceramide	Chemical		metabolized to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_8_1244_s_345	12177168	Our results indicate that it is unlikely that PLD activation by ATP is mediated by ceramide or its possible metabolism to sphingosine or sphingosine 1-phosphate, as ATP does not cause ceramide accumulation in the acini.	transcription
59505	4	335943	5	NULL	NULL	0	NULL	statement 3	Process		does not mediate					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_8_1244_s_345	12177168	Our results indicate that it is unlikely that PLD activation by ATP is mediated by ceramide or its possible metabolism to sphingosine or sphingosine 1-phosphate, as ATP does not cause ceramide accumulation in the acini.	transcription
59506	5	335943	5	NULL	NULL	0	NULL	ceramide	Chemical		metabolized to					sphingosine 1-phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_8_1244_s_345	12177168	Our results indicate that it is unlikely that PLD activation by ATP is mediated by ceramide or its possible metabolism to sphingosine or sphingosine 1-phosphate, as ATP does not cause ceramide accumulation in the acini.	transcription
59507	6	335943	5	NULL	NULL	0	NULL	statement 5	Process		does not mediate					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_8_1244_s_345	12177168	Our results indicate that it is unlikely that PLD activation by ATP is mediated by ceramide or its possible metabolism to sphingosine or sphingosine 1-phosphate, as ATP does not cause ceramide accumulation in the acini.	transcription
59508	7	335943	5	NULL	NULL	0	NULL	ATP	Chemical		does not cause					ceramide	Chemical	accumulation of			NULL	acini	NULL	NULL	NULL	NULL	gw60_jlipidres_43_8_1244_s_345	12177168	Our results indicate that it is unlikely that PLD activation by ATP is mediated by ceramide or its possible metabolism to sphingosine or sphingosine 1-phosphate, as ATP does not cause ceramide accumulation in the acini.	transcription
79314	1	335943	6	NULL	NULL	0	NULL	ATP	Chemical		activates					PLD	GP				NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_8_1244_s_345	12177168	Our results indicate that it is unlikely that PLD activation by ATP is mediated by ceramide or its possible metabolism to sphingosine or sphingosine 1-phosphate, as ATP does not cause ceramide accumulation in the acini.	transcription
79315	2	335943	6	NULL	NULL	0	NULL	ATP	Chemical		does not cause					ceramide	Chemical	accumulation of 			NULL	acini	0	NULL	NULL	NULL	gw60_jlipidres_43_8_1244_s_345	12177168	Our results indicate that it is unlikely that PLD activation by ATP is mediated by ceramide or its possible metabolism to sphingosine or sphingosine 1-phosphate, as ATP does not cause ceramide accumulation in the acini.	transcription
59509	1	335944	5	NULL	NULL	0	NULL	TNF-alpha	GP		signals					cell death	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_30_27879_s_2	15946935	umor necrosis factor (TNF)-alpha signals cell death and simultaneously induces the generation of ceramide, which is metabolized to sphingosine and sphingosine 1-phosphate (S1P) by ceramidase (CDase) and sphingosine kinase.	transcription
59510	2	335944	5	NULL	NULL	0	NULL	TNF	GP		is					tumor necrosis factor	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_30_27879_s_2	15946935	umor necrosis factor (TNF)-alpha signals cell death and simultaneously induces the generation of ceramide, which is metabolized to sphingosine and sphingosine 1-phosphate (S1P) by ceramidase (CDase) and sphingosine kinase.	transcription
59511	3	335944	5	NULL	NULL	0	NULL	TNF-alpha	GP		induce					ceramide	Chemical	generation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_30_27879_s_2	15946935	umor necrosis factor (TNF)-alpha signals cell death and simultaneously induces the generation of ceramide, which is metabolized to sphingosine and sphingosine 1-phosphate (S1P) by ceramidase (CDase) and sphingosine kinase.	transcription
59512	4	335944	5	NULL	NULL	0	NULL	statement 1	Process		occurs simultaneously with					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_30_27879_s_2	15946935	umor necrosis factor (TNF)-alpha signals cell death and simultaneously induces the generation of ceramide, which is metabolized to sphingosine and sphingosine 1-phosphate (S1P) by ceramidase (CDase) and sphingosine kinase.	transcription
59513	5	335944	5	NULL	NULL	0	NULL	ceramide	Chemical		metabolized to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_30_27879_s_2	15946935	umor necrosis factor (TNF)-alpha signals cell death and simultaneously induces the generation of ceramide, which is metabolized to sphingosine and sphingosine 1-phosphate (S1P) by ceramidase (CDase) and sphingosine kinase.	transcription
59514	6	335944	5	NULL	NULL	0	NULL	ceramidase	GP		catalyzes					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_30_27879_s_2	15946935	umor necrosis factor (TNF)-alpha signals cell death and simultaneously induces the generation of ceramide, which is metabolized to sphingosine and sphingosine 1-phosphate (S1P) by ceramidase (CDase) and sphingosine kinase.	transcription
59515	7	335944	5	NULL	NULL	0	NULL	ceramide	Chemical		metabolized to					sphingosine 1-phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_30_27879_s_2	15946935	umor necrosis factor (TNF)-alpha signals cell death and simultaneously induces the generation of ceramide, which is metabolized to sphingosine and sphingosine 1-phosphate (S1P) by ceramidase (CDase) and sphingosine kinase.	transcription
59516	8	335944	5	NULL	NULL	0	NULL	sphingosine kinase	GP		catalyzes					statement 7	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_30_27879_s_2	15946935	umor necrosis factor (TNF)-alpha signals cell death and simultaneously induces the generation of ceramide, which is metabolized to sphingosine and sphingosine 1-phosphate (S1P) by ceramidase (CDase) and sphingosine kinase.	transcription
59517	9	335944	5	NULL	NULL	0	NULL	S1P	Chemical		is					sphingosine 1-phosphate	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_30_27879_s_2	15946935	umor necrosis factor (TNF)-alpha signals cell death and simultaneously induces the generation of ceramide, which is metabolized to sphingosine and sphingosine 1-phosphate (S1P) by ceramidase (CDase) and sphingosine kinase.	transcription
59518	10	335944	5	NULL	NULL	0	NULL	CDase	GP		is					ceramidase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_30_27879_s_2	15946935	umor necrosis factor (TNF)-alpha signals cell death and simultaneously induces the generation of ceramide, which is metabolized to sphingosine and sphingosine 1-phosphate (S1P) by ceramidase (CDase) and sphingosine kinase.	transcription
59519	1	335945	5	NULL	NULL	0	NULL	protein kinase C	GP	activation of	activates					sphingosine kinase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_289	10747891	Interestingly, activation of protein kinase C can lead to the activation of sphingosine kinase ( 91), the enzyme responsible for the conversion of sphingosine into sphingosine 1-phosphate, a sphingolipid metabolite known to antagonize ceramide-mediated apoptosis ( 35,  37,  91-93).	transcription
59520	2	335945	5	NULL	NULL	0	NULL	sphingosine	Chemical		is converted to					sphingosine 1-phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_289	10747891	Interestingly, activation of protein kinase C can lead to the activation of sphingosine kinase ( 91), the enzyme responsible for the conversion of sphingosine into sphingosine 1-phosphate, a sphingolipid metabolite known to antagonize ceramide-mediated apoptosis ( 35,  37,  91-93).	transcription
59521	3	335945	5	NULL	NULL	0	NULL	sphingosine kinase	GP		catalyzes					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_289	10747891	Interestingly, activation of protein kinase C can lead to the activation of sphingosine kinase ( 91), the enzyme responsible for the conversion of sphingosine into sphingosine 1-phosphate, a sphingolipid metabolite known to antagonize ceramide-mediated apoptosis ( 35,  37,  91-93).	transcription
59522	4	335945	5	NULL	NULL	0	NULL	sphingosine 1-phosphate	Chemical		is a metabolite of					sphingolipid	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_289	10747891	Interestingly, activation of protein kinase C can lead to the activation of sphingosine kinase ( 91), the enzyme responsible for the conversion of sphingosine into sphingosine 1-phosphate, a sphingolipid metabolite known to antagonize ceramide-mediated apoptosis ( 35,  37,  91-93).	transcription
59523	5	335945	5	NULL	NULL	0	NULL	apoptosis	Process		is mediated by					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_289	10747891	Interestingly, activation of protein kinase C can lead to the activation of sphingosine kinase ( 91), the enzyme responsible for the conversion of sphingosine into sphingosine 1-phosphate, a sphingolipid metabolite known to antagonize ceramide-mediated apoptosis ( 35,  37,  91-93).	transcription
59524	6	335945	5	NULL	NULL	0	NULL	sphingosine 1-phosphate	Chemical		antagonize					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_289	10747891	Interestingly, activation of protein kinase C can lead to the activation of sphingosine kinase ( 91), the enzyme responsible for the conversion of sphingosine into sphingosine 1-phosphate, a sphingolipid metabolite known to antagonize ceramide-mediated apoptosis ( 35,  37,  91-93).	transcription
79311	1	335945	6	NULL	NULL	0	NULL	protein kinase C	GP	activation of	activates					sphingosine kinase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_289	10747891	Interestingly, activation of protein kinase C can lead to the activation of sphingosine kinase ( 91), the enzyme responsible for the conversion of sphingosine into sphingosine 1-phosphate, a sphingolipid metabolite known to antagonize ceramide-mediated apoptosis ( 35,  37,  91-93).	transcription
79312	2	335945	6	NULL	NULL	0	NULL	sphingosine	GP		is converted to					sphingosine 1-phosphate	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_289	10747891	Interestingly, activation of protein kinase C can lead to the activation of sphingosine kinase ( 91), the enzyme responsible for the conversion of sphingosine into sphingosine 1-phosphate, a sphingolipid metabolite known to antagonize ceramide-mediated apoptosis ( 35,  37,  91-93).	transcription
79313	3	335945	6	NULL	NULL	0	NULL	sphingosine kinase	GP		catalyzes					statement 2					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_289	10747891	Interestingly, activation of protein kinase C can lead to the activation of sphingosine kinase ( 91), the enzyme responsible for the conversion of sphingosine into sphingosine 1-phosphate, a sphingolipid metabolite known to antagonize ceramide-mediated apoptosis ( 35,  37,  91-93).	transcription
59525	1	335946	5	NULL	NULL	0	NULL	fumonisin B	GP		is an inhibitor of					N-acyltransferase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_22_13541_s_123	7768956	Futhermore, in support  of ceramide as the mediator, the sphingosine  N-acyltransferase  inhibitor fumonisin B   inhibited sphingosine acylation and  blocked sphingosine-induced GVBD without affecting progesterone-induced  GVBD.	transcription
59526	2	335946	5	NULL	NULL	0	NULL	fumonisin B	GP		inhibits					sphingosine	Chemical	acylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_22_13541_s_123	7768956	Futhermore, in support  of ceramide as the mediator, the sphingosine  N-acyltransferase  inhibitor fumonisin B   inhibited sphingosine acylation and  blocked sphingosine-induced GVBD without affecting progesterone-induced  GVBD.	transcription
59527	3	335946	5	NULL	NULL	0	NULL	sphingosine	Chemical		induce					GVBD	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_22_13541_s_123	7768956	Futhermore, in support  of ceramide as the mediator, the sphingosine  N-acyltransferase  inhibitor fumonisin B   inhibited sphingosine acylation and  blocked sphingosine-induced GVBD without affecting progesterone-induced  GVBD.	transcription
59528	4	335946	5	NULL	NULL	0	NULL	fumonisin B	GP		blocks					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_22_13541_s_123	7768956	Futhermore, in support  of ceramide as the mediator, the sphingosine  N-acyltransferase  inhibitor fumonisin B   inhibited sphingosine acylation and  blocked sphingosine-induced GVBD without affecting progesterone-induced  GVBD.	transcription
59529	5	335946	5	NULL	NULL	0	NULL	progesterone	GP		induce					GVBD	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_22_13541_s_123	7768956	Futhermore, in support  of ceramide as the mediator, the sphingosine  N-acyltransferase  inhibitor fumonisin B   inhibited sphingosine acylation and  blocked sphingosine-induced GVBD without affecting progesterone-induced  GVBD.	transcription
59530	6	335946	5	NULL	NULL	0	NULL	statement 4	Process		does not affect					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_22_13541_s_123	7768956	Futhermore, in support  of ceramide as the mediator, the sphingosine  N-acyltransferase  inhibitor fumonisin B   inhibited sphingosine acylation and  blocked sphingosine-induced GVBD without affecting progesterone-induced  GVBD.	transcription
79306	1	335946	6	NULL	NULL	0	NULL	sphingosine N-acyltransferase inhibitor	GP		inhibits					sphingosine	Chemical	acylation of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_22_13541_s_123	7768956	Futhermore, in support  of ceramide as the mediator, the sphingosine  N-acyltransferase  inhibitor fumonisin B   inhibited sphingosine acylation and  blocked sphingosine-induced GVBD without affecting progesterone-induced  GVBD.	transcription
79307	2	335946	6	NULL	NULL	0	NULL	sphingosine	Chemical		induces					GVBD	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_22_13541_s_123	7768956	Futhermore, in support  of ceramide as the mediator, the sphingosine  N-acyltransferase  inhibitor fumonisin B   inhibited sphingosine acylation and  blocked sphingosine-induced GVBD without affecting progesterone-induced  GVBD.	transcription
79308	3	335946	6	NULL	NULL	0	NULL	progesterone	GP		induces					GVBD	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_22_13541_s_123	7768956	Futhermore, in support  of ceramide as the mediator, the sphingosine  N-acyltransferase  inhibitor fumonisin B   inhibited sphingosine acylation and  blocked sphingosine-induced GVBD without affecting progesterone-induced  GVBD.	transcription
79309	4	335946	6	NULL	NULL	0	NULL	fumonisin B	Chemical		inhibits					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_22_13541_s_123	7768956	Futhermore, in support  of ceramide as the mediator, the sphingosine  N-acyltransferase  inhibitor fumonisin B   inhibited sphingosine acylation and  blocked sphingosine-induced GVBD without affecting progesterone-induced  GVBD.	transcription
79310	5	335946	6	NULL	NULL	0	NULL	fumonisin B	Chemical		is a type of					sphingosine N-acyltransferase inhibitor	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_22_13541_s_123	7768956	Futhermore, in support  of ceramide as the mediator, the sphingosine  N-acyltransferase  inhibitor fumonisin B   inhibited sphingosine acylation and  blocked sphingosine-induced GVBD without affecting progesterone-induced  GVBD.	transcription
59531	1	335947	5	NULL	NULL	0	NULL	sphingosine	Chemical		induce					SMC	Cell	proliferation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_31_21533_s_183	10419457	Last, sphingosine-induced SMC proliferation was not blocked by FB1 (155  plus-or-minus  7%) (data not shown), indicating that re-acylation of sphingosine to ceramide is not required for the effect of sphingosine.	transcription
59532	2	335947	5	NULL	NULL	0	NULL	FB1	GP		does not block					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_31_21533_s_183	10419457	Last, sphingosine-induced SMC proliferation was not blocked by FB1 (155  plus-or-minus  7%) (data not shown), indicating that re-acylation of sphingosine to ceramide is not required for the effect of sphingosine.	transcription
59533	3	335947	5	NULL	NULL	0	NULL	sphingosine	Chemical		is re-acylated to					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_31_21533_s_183	10419457	Last, sphingosine-induced SMC proliferation was not blocked by FB1 (155  plus-or-minus  7%) (data not shown), indicating that re-acylation of sphingosine to ceramide is not required for the effect of sphingosine.	transcription
59534	4	335947	5	NULL	NULL	0	NULL	statement 3	Process		is not required for					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_31_21533_s_183	10419457	Last, sphingosine-induced SMC proliferation was not blocked by FB1 (155  plus-or-minus  7%) (data not shown), indicating that re-acylation of sphingosine to ceramide is not required for the effect of sphingosine.	transcription
79304	1	335947	6	NULL	NULL	0	NULL	sphingosine	Chemical		induces					SMC	cell	proliferation of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_31_21533_s_183	10419457	Last, sphingosine-induced SMC proliferation was not blocked by FB1 (155  plus-or-minus  7%) (data not shown), indicating that re-acylation of sphingosine to ceramide is not required for the effect of sphingosine.	transcription
79305	2	335947	6	NULL	NULL	0	NULL	statement 1	Process		is not blocked by					FB1	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_31_21533_s_183	10419457	Last, sphingosine-induced SMC proliferation was not blocked by FB1 (155  plus-or-minus  7%) (data not shown), indicating that re-acylation of sphingosine to ceramide is not required for the effect of sphingosine.	transcription
59535	1	335948	5	NULL	NULL	0	NULL	ceramide	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_28_26577_s_316	11356846	It has been shown that both ceramide and its intermediate breakdown product sphingosine induce apoptosis or growth suppression of many cancerous cell lines ( 36-38), whereas its subsequent product sphingosine-1-P has a proliferative effect on fibroblast or endothelial cells ( 39).	transcription
59536	2	335948	5	NULL	NULL	0	NULL	sphingosine	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_28_26577_s_316	11356846	It has been shown that both ceramide and its intermediate breakdown product sphingosine induce apoptosis or growth suppression of many cancerous cell lines ( 36-38), whereas its subsequent product sphingosine-1-P has a proliferative effect on fibroblast or endothelial cells ( 39).	transcription
59537	3	335948	5	NULL	NULL	0	NULL	ceramide	Chemical		suppress					cancerous cell lines	Cell	growth of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_28_26577_s_316	11356846	It has been shown that both ceramide and its intermediate breakdown product sphingosine induce apoptosis or growth suppression of many cancerous cell lines ( 36-38), whereas its subsequent product sphingosine-1-P has a proliferative effect on fibroblast or endothelial cells ( 39).	transcription
59538	4	335948	5	NULL	NULL	0	NULL	sphingosine	Chemical		suppress					cancerous cell lines	Cell	growth of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_28_26577_s_316	11356846	It has been shown that both ceramide and its intermediate breakdown product sphingosine induce apoptosis or growth suppression of many cancerous cell lines ( 36-38), whereas its subsequent product sphingosine-1-P has a proliferative effect on fibroblast or endothelial cells ( 39).	transcription
59539	5	335948	5	NULL	NULL	0	NULL	sphingosine	Chemical		is a breakdown product of		intermediate			ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_28_26577_s_316	11356846	It has been shown that both ceramide and its intermediate breakdown product sphingosine induce apoptosis or growth suppression of many cancerous cell lines ( 36-38), whereas its subsequent product sphingosine-1-P has a proliferative effect on fibroblast or endothelial cells ( 39).	transcription
59540	6	335948	5	NULL	NULL	0	NULL	sphingosine-1-P	Chemical		proliferates					fibroblast	Cell				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_28_26577_s_316	11356846	It has been shown that both ceramide and its intermediate breakdown product sphingosine induce apoptosis or growth suppression of many cancerous cell lines ( 36-38), whereas its subsequent product sphingosine-1-P has a proliferative effect on fibroblast or endothelial cells ( 39).	transcription
59541	7	335948	5	NULL	NULL	0	NULL	sphingosine 1-phosphate	Chemical		proliferates					endothelial cells	Cell				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_28_26577_s_316	11356846	It has been shown that both ceramide and its intermediate breakdown product sphingosine induce apoptosis or growth suppression of many cancerous cell lines ( 36-38), whereas its subsequent product sphingosine-1-P has a proliferative effect on fibroblast or endothelial cells ( 39).	transcription
79300	1	335948	6	NULL	NULL	0	NULL	ceramide	Chemical		induces					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_28_26577_s_316	11356846	It has been shown that both ceramide and its intermediate breakdown product sphingosine induce apoptosis or growth suppression of many cancerous cell lines ( 36-38), whereas its subsequent product sphingosine-1-P has a proliferative effect on fibroblast or endothelial cells ( 39).	transcription
79301	2	335948	6	NULL	NULL	0	NULL	sphingosine	Chemical		induces					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_28_26577_s_316	11356846	It has been shown that both ceramide and its intermediate breakdown product sphingosine induce apoptosis or growth suppression of many cancerous cell lines ( 36-38), whereas its subsequent product sphingosine-1-P has a proliferative effect on fibroblast or endothelial cells ( 39).	transcription
79302	3	335948	6	NULL	NULL	0	NULL	sphingosine-1-P	GP		proliferates					fibroblast cells	cell				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_28_26577_s_316	11356846	It has been shown that both ceramide and its intermediate breakdown product sphingosine induce apoptosis or growth suppression of many cancerous cell lines ( 36-38), whereas its subsequent product sphingosine-1-P has a proliferative effect on fibroblast or endothelial cells ( 39).	transcription
79303	4	335948	6	NULL	NULL	0	NULL	sphingosine-1 phosphate	GP		proliferates					endothelial cells	Cell				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_28_26577_s_316	11356846	It has been shown that both ceramide and its intermediate breakdown product sphingosine induce apoptosis or growth suppression of many cancerous cell lines ( 36-38), whereas its subsequent product sphingosine-1-P has a proliferative effect on fibroblast or endothelial cells ( 39).	transcription
59542	1	335949	5	NULL	NULL	0	NULL	S1P	Chemical		regulates					cellular growth	Process				NULL		0	NULL	NULL	NULL	gw70_biolreprod_70_3_759_s_24	14613902	In contrast with the growth-inhibitory and proapoptotic actions of ceramide and sphingosine, S1P regulates diverse processes such as cellular growth, inhibition of ceramide-mediated apoptosis, and cell migration [ ].	transcription
59543	2	335949	5	NULL	NULL	0	NULL	ceramide	Chemical		mediates					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw70_biolreprod_70_3_759_s_24	14613902	In contrast with the growth-inhibitory and proapoptotic actions of ceramide and sphingosine, S1P regulates diverse processes such as cellular growth, inhibition of ceramide-mediated apoptosis, and cell migration [ ].	transcription
59544	3	335949	5	NULL	NULL	0	NULL	S1P	Chemical		regulates					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_biolreprod_70_3_759_s_24	14613902	In contrast with the growth-inhibitory and proapoptotic actions of ceramide and sphingosine, S1P regulates diverse processes such as cellular growth, inhibition of ceramide-mediated apoptosis, and cell migration [ ].	transcription
59545	4	335949	5	NULL	NULL	0	NULL	S1P	Chemical		regulates					cell migration	Process				NULL		0	NULL	NULL	NULL	gw70_biolreprod_70_3_759_s_24	14613902	In contrast with the growth-inhibitory and proapoptotic actions of ceramide and sphingosine, S1P regulates diverse processes such as cellular growth, inhibition of ceramide-mediated apoptosis, and cell migration [ ].	transcription
79296	1	335949	6	NULL	NULL	0	NULL	S1p	GP		regulates					cell growth	Process				NULL		0	NULL	NULL	NULL	gw70_biolreprod_70_3_759_s_24	14613902	In contrast with the growth-inhibitory and proapoptotic actions of ceramide and sphingosine, S1P regulates diverse processes such as cellular growth, inhibition of ceramide-mediated apoptosis, and cell migration [ ].	transcription
79297	2	335949	6	NULL	NULL	0	NULL	S1P	GP		regulates					cell migration	Process				NULL		0	NULL	NULL	NULL	gw70_biolreprod_70_3_759_s_24	14613902	In contrast with the growth-inhibitory and proapoptotic actions of ceramide and sphingosine, S1P regulates diverse processes such as cellular growth, inhibition of ceramide-mediated apoptosis, and cell migration [ ].	transcription
79298	3	335949	6	NULL	NULL	0	NULL	ceramide	Chemical		mediates					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw70_biolreprod_70_3_759_s_24	14613902	In contrast with the growth-inhibitory and proapoptotic actions of ceramide and sphingosine, S1P regulates diverse processes such as cellular growth, inhibition of ceramide-mediated apoptosis, and cell migration [ ].	transcription
79299	4	335949	6	NULL	NULL	0	NULL	S1P	GP		regulates					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_biolreprod_70_3_759_s_24	14613902	In contrast with the growth-inhibitory and proapoptotic actions of ceramide and sphingosine, S1P regulates diverse processes such as cellular growth, inhibition of ceramide-mediated apoptosis, and cell migration [ ].	transcription
59546	1	335950	5	NULL	NULL	0	NULL	ceramide	Chemical		induce					cell death	Process				NULL	sensory neurons	0	NULL	NULL	NULL	gw70_neuropharmacology_45_8_1130_s_998	14614956	S.E. Ping and G.L. Barrett, Ceramide can induce cell death in sensory neurons, whereas  ceramide analogues and sphingosine promote survival.	transcription
59547	2	335950	5	NULL	NULL	0	NULL	ceramide analogues	Chemical		promotes					cell survival	Process				NULL	sensory neurons	0	NULL	NULL	NULL	gw70_neuropharmacology_45_8_1130_s_998	14614956	S.E. Ping and G.L. Barrett, Ceramide can induce cell death in sensory neurons, whereas  ceramide analogues and sphingosine promote survival.	transcription
59548	3	335950	5	NULL	NULL	0	NULL	sphingosine	Chemical		promotes					cell survival	Process				NULL	sensory neurons	0	NULL	NULL	NULL	gw70_neuropharmacology_45_8_1130_s_998	14614956	S.E. Ping and G.L. Barrett, Ceramide can induce cell death in sensory neurons, whereas  ceramide analogues and sphingosine promote survival.	transcription
79294	1	335950	6	NULL	NULL	0	NULL	ceramide	Chemical		induces					cell death	Process				NULL	sensory neurons	0	NULL	NULL	NULL	gw70_neuropharmacology_45_8_1130_s_998	14614956	S.E. Ping and G.L. Barrett, Ceramide can induce cell death in sensory neurons, whereas  ceramide analogues and sphingosine promote survival.	transcription
79295	2	335950	6	NULL	NULL	0	NULL	sphingosine	Chemical		promotes					cell survival	Process				NULL		0	NULL	NULL	NULL	gw70_neuropharmacology_45_8_1130_s_998	14614956	S.E. Ping and G.L. Barrett, Ceramide can induce cell death in sensory neurons, whereas  ceramide analogues and sphingosine promote survival.	transcription
59549	1	335951	5	NULL	NULL	0	NULL	ceramide	Chemical	natural	induce					c-jun	GP				NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_75	12135749	Because the time-course of c-jun induction by natural ceramide was much slower than that by sphingosine or C2-ceramide, natural ceramide was not used in the experiments described below.	transcription
59550	2	335951	5	NULL	NULL	0	NULL	sphingosine	Chemical		induce					c-jun	GP				NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_75	12135749	Because the time-course of c-jun induction by natural ceramide was much slower than that by sphingosine or C2-ceramide, natural ceramide was not used in the experiments described below.	transcription
59551	3	335951	5	NULL	NULL	0	NULL	C2-ceramide	Chemical		induce					c-jun	GP				NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_75	12135749	Because the time-course of c-jun induction by natural ceramide was much slower than that by sphingosine or C2-ceramide, natural ceramide was not used in the experiments described below.	transcription
59552	4	335951	5	NULL	NULL	0	NULL	statement 1	Process		slower than					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_75	12135749	Because the time-course of c-jun induction by natural ceramide was much slower than that by sphingosine or C2-ceramide, natural ceramide was not used in the experiments described below.	transcription
59553	5	335951	5	NULL	NULL	0	NULL	statement 1	Process		slower than					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_75	12135749	Because the time-course of c-jun induction by natural ceramide was much slower than that by sphingosine or C2-ceramide, natural ceramide was not used in the experiments described below.	transcription
59554	1	335952	5	NULL	NULL	0	NULL	ceramide	Chemical		stimulates					epidermal growth factor receptor	GP	phosphorylation of			NULL	A431 cells	0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_476	9415703	Ceramide stimulates epidermal growth factor receptor phosphorylation in A431 human epidermoid carcinoma cells: evidence that ceramide may mediate sphingosine action.	transcription
59555	2	335952	5	NULL	NULL	0	NULL	A431 cells	Cell		is					human epidermoid carcinoma cells	Cell				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_476	9415703	Ceramide stimulates epidermal growth factor receptor phosphorylation in A431 human epidermoid carcinoma cells: evidence that ceramide may mediate sphingosine action.	transcription
59556	3	335952	5	NULL	NULL	0	NULL	ceramide	Chemical		mediates		may			sphingosine	Chemical	action of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_476	9415703	Ceramide stimulates epidermal growth factor receptor phosphorylation in A431 human epidermoid carcinoma cells: evidence that ceramide may mediate sphingosine action.	transcription
79292	1	335952	6	NULL	NULL	0	NULL	ceramide	Chemical		stimulates					epidermal growth factor receptor	GP	phosphorylation of			NULL	A431 human epidermoid carcinoma cells	0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_476	9415703	Ceramide stimulates epidermal growth factor receptor phosphorylation in A431 human epidermoid carcinoma cells: evidence that ceramide may mediate sphingosine action.	transcription
79293	2	335952	6	NULL	NULL	0	NULL	ceramide	Chemical		mediates					sphingosine	Chemical	action of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_476	9415703	Ceramide stimulates epidermal growth factor receptor phosphorylation in A431 human epidermoid carcinoma cells: evidence that ceramide may mediate sphingosine action.	transcription
59557	1	335953	5	NULL	NULL	0	NULL	ceramide	Chemical		is a type of					sphingolipid	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_29_27129_s_188	11369765	To determine whether sphingolipids such as ceramide and sphingosine could affect the accumulation of p53, LM cells were treated with ceramide, and their cellular p53 protein levels were measured.	transcription
59558	2	335953	5	NULL	NULL	0	NULL	sphingosine	Chemical		is a type of					sphingolipid	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_27129_s_188	11369765	To determine whether sphingolipids such as ceramide and sphingosine could affect the accumulation of p53, LM cells were treated with ceramide, and their cellular p53 protein levels were measured.	transcription
59559	3	335953	5	NULL	NULL	0	NULL	ceramide	Chemical		affects		may			p53	GP	accumulation of			NULL	LM cells	0	NULL	NULL	NULL	gw60_jbiolchem_276_29_27129_s_188	11369765	To determine whether sphingolipids such as ceramide and sphingosine could affect the accumulation of p53, LM cells were treated with ceramide, and their cellular p53 protein levels were measured.	transcription
59560	4	335953	5	NULL	NULL	0	NULL	sphingosine	Chemical		affects		may			p53	GP	accumulation of			NULL	LM cells	0	NULL	NULL	NULL	gw60_jbiolchem_276_29_27129_s_188	11369765	To determine whether sphingolipids such as ceramide and sphingosine could affect the accumulation of p53, LM cells were treated with ceramide, and their cellular p53 protein levels were measured.	transcription
59561	1	335954	5	NULL	NULL	0	NULL	ceramide	Chemical		is an inhibitor of		potent			PLD	GP	activity of			NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_8_1244_s_344	12177168	Although ceramides are potent inhibitors of PLD activity in a variety of cell types ( 13,  14,  18,  26,  28,  30 -  33), in human fibroblasts, ceramides or sphingosine can activate PLD ( 34).	transcription
59562	2	335954	5	NULL	NULL	0	NULL	ceramide	Chemical		activates					PLD	GP				NULL	human fibroblasts	0	NULL	NULL	NULL	gw60_jlipidres_43_8_1244_s_344	12177168	Although ceramides are potent inhibitors of PLD activity in a variety of cell types ( 13,  14,  18,  26,  28,  30 -  33), in human fibroblasts, ceramides or sphingosine can activate PLD ( 34).	transcription
59563	3	335954	5	NULL	NULL	0	NULL	sphingosine	Chemical		activates					PLD	GP				NULL	human fibroblasts	0	NULL	NULL	NULL	gw60_jlipidres_43_8_1244_s_344	12177168	Although ceramides are potent inhibitors of PLD activity in a variety of cell types ( 13,  14,  18,  26,  28,  30 -  33), in human fibroblasts, ceramides or sphingosine can activate PLD ( 34).	transcription
59564	4	335954	5	NULL	NULL	0	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_8_1244_s_344	12177168	Although ceramides are potent inhibitors of PLD activity in a variety of cell types ( 13,  14,  18,  26,  28,  30 -  33), in human fibroblasts, ceramides or sphingosine can activate PLD ( 34).	transcription
79291	1	335954	6	NULL	NULL	0	NULL	ceramide	Chemical		inhibits					PLD activity	Process				NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_8_1244_s_344	12177168	Although ceramides are potent inhibitors of PLD activity in a variety of cell types ( 13,  14,  18,  26,  28,  30 -  33), in human fibroblasts, ceramides or sphingosine can activate PLD ( 34).	transcription
59565	1	335955	5	NULL	NULL	0	NULL	ceramide	Chemical		mediates					programmed cell death	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_54_1_70_s_247	9658191	Cuvillier O, Pirianov G, Kleuser B, Vanek PG, Coso OA, Gutkind S and Spiegel S (1996) Suppression of ceramide-mediated programmed cell death by sphingosine-1 phosphate.	transcription
59566	2	335955	5	NULL	NULL	0	NULL	sphingosine 1-phosphate	Chemical		suppress					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_54_1_70_s_247	9658191	Cuvillier O, Pirianov G, Kleuser B, Vanek PG, Coso OA, Gutkind S and Spiegel S (1996) Suppression of ceramide-mediated programmed cell death by sphingosine-1 phosphate.	transcription
79289	1	335955	6	NULL	NULL	0	NULL	ceramide	Chemical		mediates					programmed cell death	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_54_1_70_s_247	9658191	Cuvillier O, Pirianov G, Kleuser B, Vanek PG, Coso OA, Gutkind S and Spiegel S (1996) Suppression of ceramide-mediated programmed cell death by sphingosine-1 phosphate.	transcription
79290	2	335955	6	NULL	NULL	0	NULL	sphingosine-1 phosphate	GP		suppresses					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_54_1_70_s_247	9658191	Cuvillier O, Pirianov G, Kleuser B, Vanek PG, Coso OA, Gutkind S and Spiegel S (1996) Suppression of ceramide-mediated programmed cell death by sphingosine-1 phosphate.	transcription
59567	1	335956	5	NULL	NULL	0	NULL	JNK	GP		is activated by					TNF	GP				NULL		0	NULL	NULL	NULL	gw70_intjdevneurosci_19_4_427_s_259	11378302	Other studies have confirmed the activation of JNK by TNF- , as well as by ceramide,  sphingosine and sphingomyelinase (  Fig. 2).	transcription
59568	2	335956	5	NULL	NULL	0	NULL	JNK	GP		is activated by					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw70_intjdevneurosci_19_4_427_s_259	11378302	Other studies have confirmed the activation of JNK by TNF- , as well as by ceramide,  sphingosine and sphingomyelinase (  Fig. 2).	transcription
59569	3	335956	5	NULL	NULL	0	NULL	JNK	GP		is activated by					sphingosine	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_intjdevneurosci_19_4_427_s_259	11378302	Other studies have confirmed the activation of JNK by TNF- , as well as by ceramide,  sphingosine and sphingomyelinase (  Fig. 2).	transcription
59570	4	335956	5	NULL	NULL	0	NULL	JNK	GP		is activated by					sphingomyelinase	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_intjdevneurosci_19_4_427_s_259	11378302	Other studies have confirmed the activation of JNK by TNF- , as well as by ceramide,  sphingosine and sphingomyelinase (  Fig. 2).	transcription
79285	1	335956	6	NULL	NULL	0	NULL	TNF	GP		activates					JNK	GP				NULL		0	NULL	NULL	NULL	gw70_intjdevneurosci_19_4_427_s_259	11378302	Other studies have confirmed the activation of JNK by TNF- , as well as by ceramide,  sphingosine and sphingomyelinase (  Fig. 2).	transcription
79286	2	335956	6	NULL	NULL	0	NULL	ceramide	Chemical		activates					JNK	GP				NULL		0	NULL	NULL	NULL	gw70_intjdevneurosci_19_4_427_s_259	11378302	Other studies have confirmed the activation of JNK by TNF- , as well as by ceramide,  sphingosine and sphingomyelinase (  Fig. 2).	transcription
79287	3	335956	6	NULL	NULL	0	NULL	sphingosine	Chemical		activates					JNK	GP				NULL		0	NULL	NULL	NULL	gw70_intjdevneurosci_19_4_427_s_259	11378302	Other studies have confirmed the activation of JNK by TNF- , as well as by ceramide,  sphingosine and sphingomyelinase (  Fig. 2).	transcription
79288	4	335956	6	NULL	NULL	0	NULL	sphingomyelinase	GP		activates					JNK	GP				NULL		0	NULL	NULL	NULL	gw70_intjdevneurosci_19_4_427_s_259	11378302	Other studies have confirmed the activation of JNK by TNF- , as well as by ceramide,  sphingosine and sphingomyelinase (  Fig. 2).	transcription
59571	1	335957	5	NULL	NULL	0	NULL	TNF-alpha	GP		is not induced by					C2 ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_194	16936207	TNF-alpha and IL-6 were not induced by C2 ceramide but were induced by sphingosine and S1P.	transcription
59572	2	335957	5	NULL	NULL	0	NULL	TNF-alpha	GP		is induced by					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_194	16936207	TNF-alpha and IL-6 were not induced by C2 ceramide but were induced by sphingosine and S1P.	transcription
59573	3	335957	5	NULL	NULL	0	NULL	TNF-alpha	GP		is induced by					S1P	Chemical				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_194	16936207	TNF-alpha and IL-6 were not induced by C2 ceramide but were induced by sphingosine and S1P.	transcription
59574	4	335957	5	NULL	NULL	0	NULL	IL-6	GP		is not induced by					C2 ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_194	16936207	TNF-alpha and IL-6 were not induced by C2 ceramide but were induced by sphingosine and S1P.	transcription
59575	5	335957	5	NULL	NULL	0	NULL	IL-6	GP		is induced by					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_194	16936207	TNF-alpha and IL-6 were not induced by C2 ceramide but were induced by sphingosine and S1P.	transcription
59576	6	335957	5	NULL	NULL	0	NULL	IL-6	GP		is induced by					S1P	Chemical				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_194	16936207	TNF-alpha and IL-6 were not induced by C2 ceramide but were induced by sphingosine and S1P.	transcription
59577	1	335959	5	NULL	NULL	0	NULL	apoptosis	Process		is mediated by					ceramide	Chemical				NULL	tumor cells	0	NULL	NULL	NULL	gw70_biolreprod_71_6_2072_s_159	15317688	Some cancer therapies are based on inhibition of sphingosine-kinase activity to amplify ceramide-mediated apoptosis in tumor cells [ ].	transcription
59578	2	335959	5	NULL	NULL	0	NULL	sphingosine-kinase	GP	inhibition of;;activity of	amplify					statement 1	Process				NULL	tumor cells	0	NULL	NULL	NULL	gw70_biolreprod_71_6_2072_s_159	15317688	Some cancer therapies are based on inhibition of sphingosine-kinase activity to amplify ceramide-mediated apoptosis in tumor cells [ ].	transcription
79277	1	335959	6	NULL	NULL	0	NULL	sphingosine-kinase activity	Process	inhibition of 	amplify					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_biolreprod_71_6_2072_s_159	15317688	Some cancer therapies are based on inhibition of sphingosine-kinase activity to amplify ceramide-mediated apoptosis in tumor cells [ ].	transcription
79278	2	335959	6	NULL	NULL	0	NULL	ceramide	Chemical		mediates					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw70_biolreprod_71_6_2072_s_159	15317688	Some cancer therapies are based on inhibition of sphingosine-kinase activity to amplify ceramide-mediated apoptosis in tumor cells [ ].	transcription
59579	1	335960	5	NULL	NULL	0	NULL	ASM	GP		is					acidic sphingomyelinase	GP				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_19_0_497_s_217	11244045	The effect requires the expression of acidic sphingomyelinase (ASM), which is activated  by CD95 stimulation to produce ceramide and its metabolite, sphingosine.	transcription
59580	2	335960	5	NULL	NULL	0	NULL	ASM	GP	expression of	is activated by					CD95	GP	stimulation of			NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_19_0_497_s_217	11244045	The effect requires the expression of acidic sphingomyelinase (ASM), which is activated  by CD95 stimulation to produce ceramide and its metabolite, sphingosine.	transcription
59581	3	335960	5	NULL	NULL	0	NULL	statement 2	Process		produce					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_19_0_497_s_217	11244045	The effect requires the expression of acidic sphingomyelinase (ASM), which is activated  by CD95 stimulation to produce ceramide and its metabolite, sphingosine.	transcription
59582	4	335960	5	NULL	NULL	0	NULL	statement 2	Process		produce					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_19_0_497_s_217	11244045	The effect requires the expression of acidic sphingomyelinase (ASM), which is activated  by CD95 stimulation to produce ceramide and its metabolite, sphingosine.	transcription
59583	5	335960	5	NULL	NULL	0	NULL	sphingosine	Chemical		is a metabolite of					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_19_0_497_s_217	11244045	The effect requires the expression of acidic sphingomyelinase (ASM), which is activated  by CD95 stimulation to produce ceramide and its metabolite, sphingosine.	transcription
79273	1	335960	6	NULL	NULL	0	NULL	ASM	Chemical		is					acidic sphingomyelinase	Chemical				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_19_0_497_s_217	11244045	The effect requires the expression of acidic sphingomyelinase (ASM), which is activated  by CD95 stimulation to produce ceramide and its metabolite, sphingosine.	transcription
79274	2	335960	6	NULL	NULL	0	NULL	CD95	GP	stimulation of 	produces					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_19_0_497_s_217	11244045	The effect requires the expression of acidic sphingomyelinase (ASM), which is activated  by CD95 stimulation to produce ceramide and its metabolite, sphingosine.	transcription
79275	3	335960	6	NULL	NULL	0	NULL	CD95	GP	stimulation of 	produces					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_19_0_497_s_217	11244045	The effect requires the expression of acidic sphingomyelinase (ASM), which is activated  by CD95 stimulation to produce ceramide and its metabolite, sphingosine.	transcription
79276	4	335960	6	NULL	NULL	0	NULL	CD95	GP		activates					ASM	Chemical				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_19_0_497_s_217	11244045	The effect requires the expression of acidic sphingomyelinase (ASM), which is activated  by CD95 stimulation to produce ceramide and its metabolite, sphingosine.	transcription
59584	1	335961	5	NULL	NULL	0	NULL	sphingosine	Chemical	addition of	stimulates					ceramide	Chemical	fomation of			NULL		0	NULL	NULL	NULL	gw70_atherosclerosis_167_1_159_s_107	12618281	Conversely the stimulation  of ceramide formation by the addition of sphingosine resulted in increased SRE mediated  transcription.	transcription
59585	2	335961	5	NULL	NULL	0	NULL	transcription	Process		is mediated by					SRE	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_atherosclerosis_167_1_159_s_107	12618281	Conversely the stimulation  of ceramide formation by the addition of sphingosine resulted in increased SRE mediated  transcription.	transcription
59586	3	335961	5	NULL	NULL	0	NULL	statement 1	Process		results in					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_atherosclerosis_167_1_159_s_107	12618281	Conversely the stimulation  of ceramide formation by the addition of sphingosine resulted in increased SRE mediated  transcription.	transcription
79271	1	335961	6	NULL	NULL	0	NULL	SRE	GP		mediates					transcription	Process				NULL		0	NULL	NULL	NULL	gw70_atherosclerosis_167_1_159_s_107	12618281	Conversely the stimulation  of ceramide formation by the addition of sphingosine resulted in increased SRE mediated  transcription.	transcription
79272	2	335961	6	NULL	NULL	0	NULL	ceramide	GP	formation by	results in					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_atherosclerosis_167_1_159_s_107	12618281	Conversely the stimulation  of ceramide formation by the addition of sphingosine resulted in increased SRE mediated  transcription.	transcription
59587	1	335962	5	NULL	NULL	0	NULL	ceramide	Chemical		induce					apoptosis	Process				NULL	sensory neurons	0	NULL	NULL	NULL	gw70_neuropharmacology_45_8_1130_s_298	14614956	In addition, ceramide induces apoptosis in sensory neurons whereas sphingosine  induces survival ( [ Ping and Barrett, 1998]).	transcription
59588	2	335962	5	NULL	NULL	0	NULL	sphingosine	Chemical		induce					cell survival	Process				NULL	sensory neurons	0	NULL	NULL	NULL	gw70_neuropharmacology_45_8_1130_s_298	14614956	In addition, ceramide induces apoptosis in sensory neurons whereas sphingosine  induces survival ( [ Ping and Barrett, 1998]).	transcription
79269	1	335962	6	NULL	NULL	0	NULL	ceramide	Chemical		induces					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw70_neuropharmacology_45_8_1130_s_298	14614956	In addition, ceramide induces apoptosis in sensory neurons whereas sphingosine  induces survival ( [ Ping and Barrett, 1998]).	transcription
79270	2	335962	6	NULL	NULL	0	NULL	sphingosine	Chemical		induces					survival	Process				NULL		0	NULL	NULL	NULL	gw70_neuropharmacology_45_8_1130_s_298	14614956	In addition, ceramide induces apoptosis in sensory neurons whereas sphingosine  induces survival ( [ Ping and Barrett, 1998]).	transcription
59589	1	335963	5	NULL	NULL	0	NULL	ceramide	Chemical	degradation of	increases		slightly			sphingosine	Chemical	level of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_17_7359_s_363	15314148	In our studies, the slight increase in the sphingosine level could also result from ceramide degradation.	transcription
79268	1	335963	6	NULL	NULL	0	NULL	ceramide	Chemical	degradation of 	results in					sphingosine	Chemical	rise of 			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_17_7359_s_363	15314148	In our studies, the slight increase in the sphingosine level could also result from ceramide degradation.	transcription
59590	1	335964	5	NULL	NULL	0	NULL	bFGF	GP		activates					eNOS	GP				NULL		0	NULL	NULL	NULL	gw70_molpharmacol_63_2_297_s_237	12527801	bFGF Activation of eNOS via Ceramide Production Does [[ Not Involve Sphingosine 1-Phosphate  Production ]].	transcription
59591	2	335964	5	NULL	NULL	0	NULL	statement 1	Process		via					ceramide	Chemical	production of			NULL		0	NULL	NULL	NULL	gw70_molpharmacol_63_2_297_s_237	12527801	bFGF Activation of eNOS via Ceramide Production Does [[ Not Involve Sphingosine 1-Phosphate  Production ]].	transcription
59592	3	335964	5	NULL	NULL	0	NULL	statement 2	Process		does not involve					sphingosine 1-phosphate	Chemical	production of			NULL		0	NULL	NULL	NULL	gw70_molpharmacol_63_2_297_s_237	12527801	bFGF Activation of eNOS via Ceramide Production Does [[ Not Involve Sphingosine 1-Phosphate  Production ]].	transcription
79266	1	335964	6	NULL	NULL	0	NULL	bFGF	GP		activates					eNOS	Chemical				NULL		0	NULL	NULL	NULL	gw70_molpharmacol_63_2_297_s_237	12527801	bFGF Activation of eNOS via Ceramide Production Does [[ Not Involve Sphingosine 1-Phosphate  Production ]].	transcription
79267	2	335964	6	NULL	NULL	0	NULL	statement 1	Process		occurs via					ceramide	Chemical	production of 			NULL		0	NULL	NULL	NULL	gw70_molpharmacol_63_2_297_s_237	12527801	bFGF Activation of eNOS via Ceramide Production Does [[ Not Involve Sphingosine 1-Phosphate  Production ]].	transcription
59593	1	335965	5	NULL	NULL	0	NULL	FFAs	Chemical		stimulates					ceramide	Chemical	de novo synthesis of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_10	15774472	Moreover, these FFAs stimulated the  de novo synthesis of ceramide and sphingosine, two sphingolipids shown previously to inhibit insulin action.	transcription
59594	2	335965	5	NULL	NULL	0	NULL	FFAs	Chemical		stimulates					sphingosine	Chemical	de novo synthesis of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_10	15774472	Moreover, these FFAs stimulated the  de novo synthesis of ceramide and sphingosine, two sphingolipids shown previously to inhibit insulin action.	transcription
59595	3	335965	5	NULL	NULL	0	NULL	ceramide	Chemical		is a type of					sphingolipid	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_10	15774472	Moreover, these FFAs stimulated the  de novo synthesis of ceramide and sphingosine, two sphingolipids shown previously to inhibit insulin action.	transcription
59596	4	335965	5	NULL	NULL	0	NULL	sphingosine	Chemical		is a type of					sphingolipid	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_10	15774472	Moreover, these FFAs stimulated the  de novo synthesis of ceramide and sphingosine, two sphingolipids shown previously to inhibit insulin action.	transcription
59597	5	335965	5	NULL	NULL	0	NULL	ceramide	Chemical		inhibit					insulin	GP	action of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_10	15774472	Moreover, these FFAs stimulated the  de novo synthesis of ceramide and sphingosine, two sphingolipids shown previously to inhibit insulin action.	transcription
59598	6	335965	5	NULL	NULL	0	NULL	sphingosine	Chemical		inhibit					insulin	GP	action of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_10	15774472	Moreover, these FFAs stimulated the  de novo synthesis of ceramide and sphingosine, two sphingolipids shown previously to inhibit insulin action.	transcription
79264	1	335965	6	NULL	NULL	0	NULL	FFA	Chemical		stimulates					ceramide	Chemical	de novo synthesis of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_10	15774472	Moreover, these FFAs stimulated the  de novo synthesis of ceramide and sphingosine, two sphingolipids shown previously to inhibit insulin action.	transcription
79265	2	335965	6	NULL	NULL	0	NULL	FFA	Chemical		stimulates					sphingosine	Chemical	de novo synthesis of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_10	15774472	Moreover, these FFAs stimulated the  de novo synthesis of ceramide and sphingosine, two sphingolipids shown previously to inhibit insulin action.	transcription
59599	1	335966	5	NULL	NULL	0	NULL	ceramide	Chemical		is hydrolyzed to					sphingosine	Chemical				NULL	lysosome	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_38	15774472	Acid ceramidase (AC) catalyzes the lysosomal hydrolysis of ceramide to sphingosine and free fatty acid ( ).	transcription
59600	2	335966	5	NULL	NULL	0	NULL	ceramide	Chemical		is hydrolyzed to					fatty acids	Chemical	free			NULL	lysosome	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_38	15774472	Acid ceramidase (AC) catalyzes the lysosomal hydrolysis of ceramide to sphingosine and free fatty acid ( ).	transcription
59601	3	335966	5	NULL	NULL	0	NULL	statement 1	Process		occurs along with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_38	15774472	Acid ceramidase (AC) catalyzes the lysosomal hydrolysis of ceramide to sphingosine and free fatty acid ( ).	transcription
59602	4	335966	5	NULL	NULL	0	NULL	AC	GP		catalyzes					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_38	15774472	Acid ceramidase (AC) catalyzes the lysosomal hydrolysis of ceramide to sphingosine and free fatty acid ( ).	transcription
59603	5	335966	5	NULL	NULL	0	NULL	AC	GP		is					acid ceramidase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_38	15774472	Acid ceramidase (AC) catalyzes the lysosomal hydrolysis of ceramide to sphingosine and free fatty acid ( ).	transcription
79262	1	335966	6	NULL	NULL	0	NULL	ceramide	Chemical		is converted to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_38	15774472	Acid ceramidase (AC) catalyzes the lysosomal hydrolysis of ceramide to sphingosine and free fatty acid ( ).	transcription
79263	2	335966	6	NULL	NULL	0	NULL	Acid ceramidase	GP		catalyzes					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_38	15774472	Acid ceramidase (AC) catalyzes the lysosomal hydrolysis of ceramide to sphingosine and free fatty acid ( ).	transcription
59607	1	335967	5	NULL	NULL	0	NULL	AC	GP	overexpression of	prevents					ceramide	Chemical	accrual of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_40	15774472	As shown herein, overexpressing AC prevented the accrual of ceramide, but not DAG or sphingosine, induced by long-chain saturated FFAs.	transcription
59608	2	335967	5	NULL	NULL	0	NULL	AC	GP	overexpression of	does not prevent					DAG	Chemical	accrual of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_40	15774472	As shown herein, overexpressing AC prevented the accrual of ceramide, but not DAG or sphingosine, induced by long-chain saturated FFAs.	transcription
59609	3	335967	5	NULL	NULL	0	NULL	AC	GP	overexpression of	does not prevent					sphingosine	Chemical	accrual of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_40	15774472	As shown herein, overexpressing AC prevented the accrual of ceramide, but not DAG or sphingosine, induced by long-chain saturated FFAs.	transcription
59610	4	335967	5	NULL	NULL	0	NULL	ceramide	Chemical	accrual of	is induced by					FFAs	Chemical	long-chain;;saturated			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_40	15774472	As shown herein, overexpressing AC prevented the accrual of ceramide, but not DAG or sphingosine, induced by long-chain saturated FFAs.	transcription
59611	5	335967	5	NULL	NULL	0	NULL	DAG	Chemical	accrual of	is induced by					FFAs	Chemical	long-chain;;saturated 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_40	15774472	As shown herein, overexpressing AC prevented the accrual of ceramide, but not DAG or sphingosine, induced by long-chain saturated FFAs.	transcription
59612	6	335967	5	NULL	NULL	0	NULL	sphingosine	Chemical	accrual of	is induced by					FFAs	Chemical	long-chain;;saturated			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_40	15774472	As shown herein, overexpressing AC prevented the accrual of ceramide, but not DAG or sphingosine, induced by long-chain saturated FFAs.	transcription
59613	1	335968	5	NULL	NULL	0	NULL	ceramide	Chemical		is degraded to					sphingosine bases	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_4_2606_s_239	15546881	For example, sphingosine levels increase with FB1, ruling out a role for further degradation of ceramide to sphingoid bases.	transcription
59614	2	335968	5	NULL	NULL	0	NULL	sphingosine	Chemical	levels of	increase with					FB1	NucleicAcid	increase in;;levels of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_4_2606_s_239	15546881	For example, sphingosine levels increase with FB1, ruling out a role for further degradation of ceramide to sphingoid bases.	transcription
79261	1	335968	6	NULL	NULL	0	NULL	FB1	GP		increase					sphingosine 	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_4_2606_s_239	15546881	For example, sphingosine levels increase with FB1, ruling out a role for further degradation of ceramide to sphingoid bases.	transcription
59615	1	335969	5	NULL	NULL	0	NULL	SPL	GP	expression of	regulates					S1P	Chemical	intracellular			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_2_1281_s_273	14570870	First, SPL expression regulates not only intracellular S1P and sphingosine but also appears to increase ceramide generation under stress conditions.	transcription
59616	2	335969	5	NULL	NULL	0	NULL	SPL	GP	expression of	regulates					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_2_1281_s_273	14570870	First, SPL expression regulates not only intracellular S1P and sphingosine but also appears to increase ceramide generation under stress conditions.	transcription
59617	3	335969	5	NULL	NULL	0	NULL	ceramide	Chemical		is generated under					stress condition	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_2_1281_s_273	14570870	First, SPL expression regulates not only intracellular S1P and sphingosine but also appears to increase ceramide generation under stress conditions.	transcription
59618	4	335969	5	NULL	NULL	0	NULL	SPL	GP	expression of	increases					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_2_1281_s_273	14570870	First, SPL expression regulates not only intracellular S1P and sphingosine but also appears to increase ceramide generation under stress conditions.	transcription
78971	1	335969	6	NULL	NULL	0	NULL	SPL	GP	expression of	regulates					S1P	GP	intracellular			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_2_1281_s_273	14570870	First, SPL expression regulates not only intracellular S1P and sphingosine but also appears to increase ceramide generation under stress conditions.	transcription
78972	2	335969	6	NULL	NULL	0	NULL	SPL	GP	expression of	regulates					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_2_1281_s_273	14570870	First, SPL expression regulates not only intracellular S1P and sphingosine but also appears to increase ceramide generation under stress conditions.	transcription
78973	3	335969	6	NULL	NULL	0	NULL	SPL	GP	expression of	increases					ceramide	Chemical	generation of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_2_1281_s_273	14570870	First, SPL expression regulates not only intracellular S1P and sphingosine but also appears to increase ceramide generation under stress conditions.	transcription
59604	1	335970	5	NULL	NULL	0	NULL	ceramide	Chemical	hydrolysis of;;N-acyl group of	yields					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_11_7324_s_16	16380386	1.23 [EC]) catalyze the hydrolysis of the  N-acyl group of ceramide to yield sphingosine and fatty acids.	transcription
59605	2	335970	5	NULL	NULL	0	NULL	ceramide	Chemical	hydrolysis of;;N-acyl group of	yields					fatty acids	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_11_7324_s_16	16380386	1.23 [EC]) catalyze the hydrolysis of the  N-acyl group of ceramide to yield sphingosine and fatty acids.	transcription
59606	3	335970	5	NULL	NULL	0	NULL	statement 1	Process		occurs along with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_11_7324_s_16	16380386	1.23 [EC]) catalyze the hydrolysis of the  N-acyl group of ceramide to yield sphingosine and fatty acids.	transcription
78969	1	335970	6	NULL	NULL	0	NULL	ceramide	Chemical	hydrolysis of	yields			N-acyl 		sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_11_7324_s_16	16380386	1.23 [EC]) catalyze the hydrolysis of the  N-acyl group of ceramide to yield sphingosine and fatty acids.	transcription
78970	2	335970	6	NULL	NULL	0	NULL	ceramide	Chemical	hydrolysis of	yields			N-acyl 		fatty acids	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_11_7324_s_16	16380386	1.23 [EC]) catalyze the hydrolysis of the  N-acyl group of ceramide to yield sphingosine and fatty acids.	transcription
59665	1	335971	5	NULL	NULL	0	NULL	AC	GP	recombinant	catalyzes					ceramide	Chemical	synthesis of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_35_32978_s_194	12815059	We therefore evaluated whether recombinant AC could catalyze ceramide  synthesis using [14]lauric acid and sphingosine as the substrates.	transcription
59666	2	335971	5	NULL	NULL	0	NULL	lauric acid	Chemical		is a substrate of					AC	GP	recombinant			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_35_32978_s_194	12815059	We therefore evaluated whether recombinant AC could catalyze ceramide  synthesis using [14]lauric acid and sphingosine as the substrates.	transcription
59667	3	335971	5	NULL	NULL	0	NULL	sphingosine	Chemical		is a substrate of					AC	GP	recombinant			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_35_32978_s_194	12815059	We therefore evaluated whether recombinant AC could catalyze ceramide  synthesis using [14]lauric acid and sphingosine as the substrates.	transcription
59668	1	335972	5	NULL	NULL	0	NULL	ceramide	Chemical		is cleaved into					fatty acids	Chemical				NULL	normal epidermis	NULL	NULL	NULL	NULL	gw70_vetmicrobiol_99_1_67_s_139	15019113	In normal epidermis, ceramidase catalyzes the cleavage of ceramide to fatty acids  and sphingosine (  Ohnishi et al., 1999).	transcription
59669	2	335972	5	NULL	NULL	0	NULL	ceramide	Chemical		is cleaved into					sphingosine	Chemical				NULL	normal epidermis	NULL	NULL	NULL	NULL	gw70_vetmicrobiol_99_1_67_s_139	15019113	In normal epidermis, ceramidase catalyzes the cleavage of ceramide to fatty acids  and sphingosine (  Ohnishi et al., 1999).	transcription
59670	3	335972	5	NULL	NULL	0	NULL	statement 1	Process		occurs along with					statement 2	Process				NULL	normal epidermis	NULL	NULL	NULL	NULL	gw70_vetmicrobiol_99_1_67_s_139	15019113	In normal epidermis, ceramidase catalyzes the cleavage of ceramide to fatty acids  and sphingosine (  Ohnishi et al., 1999).	transcription
59671	4	335972	5	NULL	NULL	0	NULL	ceramidase	Chemical		catalyzes					statement 1	Process				NULL	normal epidermis	NULL	NULL	NULL	NULL	gw70_vetmicrobiol_99_1_67_s_139	15019113	In normal epidermis, ceramidase catalyzes the cleavage of ceramide to fatty acids  and sphingosine (  Ohnishi et al., 1999).	transcription
59672	5	335972	5	NULL	NULL	0	NULL	ceramidase	Chemical		catalyzes					statement 2	Process				NULL	normal epidermis	0	NULL	NULL	NULL	gw70_vetmicrobiol_99_1_67_s_139	15019113	In normal epidermis, ceramidase catalyzes the cleavage of ceramide to fatty acids  and sphingosine (  Ohnishi et al., 1999).	transcription
78965	1	335972	6	NULL	NULL	0	NULL	ceramide	Chemical		is cleaved to					fatty acids	Chemical				NULL		0	NULL	NULL	NULL	gw70_vetmicrobiol_99_1_67_s_139	15019113	In normal epidermis, ceramidase catalyzes the cleavage of ceramide to fatty acids  and sphingosine (  Ohnishi et al., 1999).	transcription
78966	2	335972	6	NULL	NULL	0	NULL	ceramide	Chemical		is cleaved to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_vetmicrobiol_99_1_67_s_139	15019113	In normal epidermis, ceramidase catalyzes the cleavage of ceramide to fatty acids  and sphingosine (  Ohnishi et al., 1999).	transcription
78967	3	335972	6	NULL	NULL	NULL	NULL	statement 1	Process		occurs simultaneously with					statement 2	Process				NULL	normal epidermis	NULL	NULL	NULL	NULL	gw70_vetmicrobiol_99_1_67_s_139	15019113	In normal epidermis, ceramidase catalyzes the cleavage of ceramide to fatty acids  and sphingosine (  Ohnishi et al., 1999).	transcription
78968	4	335972	6	NULL	NULL	0	NULL	ceramidase	GP		catalyzes					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_vetmicrobiol_99_1_67_s_139	15019113	In normal epidermis, ceramidase catalyzes the cleavage of ceramide to fatty acids  and sphingosine (  Ohnishi et al., 1999).	transcription
59673	1	335973	5	NULL	NULL	0	NULL	TID-ceramide	Chemical		bind					CTSD	GP				NULL		0	NULL	NULL	NULL	gw60_embo_18_19_5252_s_194	10508159	Notably, D- erythro-sphingosine, but not the fatty acid palmitate, competed for TID-ceramide binding to CTSD.	transcription
59674	2	335973	5	NULL	NULL	0	NULL	D- erythro-sphingosine	Chemical		bind					CTSD	GP				NULL		0	NULL	NULL	NULL	gw60_embo_18_19_5252_s_194	10508159	Notably, D- erythro-sphingosine, but not the fatty acid palmitate, competed for TID-ceramide binding to CTSD.	transcription
59675	3	335973	5	NULL	NULL	0	NULL	statement 2	Process		competes with					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_19_5252_s_194	10508159	Notably, D- erythro-sphingosine, but not the fatty acid palmitate, competed for TID-ceramide binding to CTSD.	transcription
59676	4	335973	5	NULL	NULL	0	NULL	palmitate	Chemical		does not compete with					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_19_5252_s_194	10508159	Notably, D- erythro-sphingosine, but not the fatty acid palmitate, competed for TID-ceramide binding to CTSD.	transcription
59677	5	335973	5	NULL	NULL	0	NULL	palmitate	Chemical		is a type of					fatty acid	Chemical				NULL		0	NULL	NULL	NULL	gw60_embo_18_19_5252_s_194	10508159	Notably, D- erythro-sphingosine, but not the fatty acid palmitate, competed for TID-ceramide binding to CTSD.	transcription
78963	1	335973	6	NULL	NULL	0	NULL	D- erythro-sphingosine	Chemical		bind					CTSD	GP				NULL		0	NULL	NULL	NULL	gw60_embo_18_19_5252_s_194	10508159	Notably, D- erythro-sphingosine, but not the fatty acid palmitate, competed for TID-ceramide binding to CTSD.	transcription
78964	2	335973	6	NULL	NULL	0	NULL	TID-ceramide	Chemical		bind					CTSD	GP				NULL		0	NULL	NULL	NULL	gw60_embo_18_19_5252_s_194	10508159	Notably, D- erythro-sphingosine, but not the fatty acid palmitate, competed for TID-ceramide binding to CTSD.	transcription
59678	1	335974	5	NULL	NULL	0	NULL	sphingosine	Chemical		is a type of					N-deacylated ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_10	12135749	Sphingosine, an  N-deacylated form of ceramide, is a potent inhibitor of protein kinase C (PKC) [  9].	transcription
59679	2	335974	5	NULL	NULL	0	NULL	sphingosine	Chemical		is an inhibitor of		potent			PKC	GP				NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_10	12135749	Sphingosine, an  N-deacylated form of ceramide, is a potent inhibitor of protein kinase C (PKC) [  9].	transcription
59680	3	335974	5	NULL	NULL	0	NULL	PKC	GP		is					protein kinase C	GP				NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_10	12135749	Sphingosine, an  N-deacylated form of ceramide, is a potent inhibitor of protein kinase C (PKC) [  9].	transcription
78960	1	335974	6	NULL	NULL	0	NULL	sphingosine	Chemical		is an inhibitor for					PKC	GP				NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_10	12135749	Sphingosine, an  N-deacylated form of ceramide, is a potent inhibitor of protein kinase C (PKC) [  9].	transcription
78961	2	335974	6	NULL	NULL	0	NULL	PKC	GP		is					protein kinase C	GP				NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_10	12135749	Sphingosine, an  N-deacylated form of ceramide, is a potent inhibitor of protein kinase C (PKC) [  9].	transcription
78962	3	335974	6	NULL	NULL	0	NULL	sphingosine	Chemical		is 					N-deacylated form of ceramide					NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_10	12135749	Sphingosine, an  N-deacylated form of ceramide, is a potent inhibitor of protein kinase C (PKC) [  9].	transcription
59681	1	335975	5	NULL	NULL	0	NULL	sphingosine	Chemical		induce					c-jun	GP	expression of			NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_83	12135749	These results suggest that sphingosine itself could induce c-jun expression and apoptosis without conversion to ceramide.	transcription
59682	2	335975	5	NULL	NULL	0	NULL	sphingosine	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_83	12135749	These results suggest that sphingosine itself could induce c-jun expression and apoptosis without conversion to ceramide.	transcription
59683	3	335975	5	NULL	NULL	0	NULL	sphingosine	Chemical		is not converted to					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_83	12135749	These results suggest that sphingosine itself could induce c-jun expression and apoptosis without conversion to ceramide.	transcription
59684	4	335975	5	NULL	NULL	0	NULL	statement 3	Process		is required for					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_83	12135749	These results suggest that sphingosine itself could induce c-jun expression and apoptosis without conversion to ceramide.	transcription
59685	5	335975	5	NULL	NULL	0	NULL	statement 3	Process		is required for					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_83	12135749	These results suggest that sphingosine itself could induce c-jun expression and apoptosis without conversion to ceramide.	transcription
78958	1	335975	6	NULL	NULL	0	NULL	sphingosine	Chemical		induces					c-jun	GP	expression of			NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_83	12135749	These results suggest that sphingosine itself could induce c-jun expression and apoptosis without conversion to ceramide.	transcription
78959	2	335975	6	NULL	NULL	0	NULL	sphingosine	Chemical		induces					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_83	12135749	These results suggest that sphingosine itself could induce c-jun expression and apoptosis without conversion to ceramide.	transcription
59704	1	335976	5	NULL	NULL	0	NULL	sphingosine	Chemical		induce					c-jun	GP	expression of			NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_142	12135749	Further studies will be needed to elucidate the signaling pathways in c-jun expression induced by sphingosine and ceramide.	transcription
59705	2	335976	5	NULL	NULL	0	NULL	ceramide	Chemical		induce					c-jun	GP	expression of			NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_142	12135749	Further studies will be needed to elucidate the signaling pathways in c-jun expression induced by sphingosine and ceramide.	transcription
78956	1	335976	6	NULL	NULL	0	NULL	sphingosine	Chemical		induces					c-jun	GP	expression of			NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_142	12135749	Further studies will be needed to elucidate the signaling pathways in c-jun expression induced by sphingosine and ceramide.	transcription
78957	2	335976	6	NULL	NULL	0	NULL	ceramide	Chemical		induces					c-jun	GP	expression of			NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_142	12135749	Further studies will be needed to elucidate the signaling pathways in c-jun expression induced by sphingosine and ceramide.	transcription
59701	1	335977	5	NULL	NULL	0	NULL	fumonisin	Chemical		is related to		structurally			sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_177_1_109_s_11	10436928	Fumonisin is structurally related to sphingosine, and FB1 is a competitive inhibitor of sphinganine  N-acyltransferase (ceramide synthase) [  12].	transcription
59702	2	335977	5	NULL	NULL	0	NULL	FB1	Chemical		is an inhibitor of		competitive			ceramide synthase	GP				NULL		NULL	NULL	NULL	NULL	gw60_femsmicrobiollett_177_1_109_s_11	10436928	Fumonisin is structurally related to sphingosine, and FB1 is a competitive inhibitor of sphinganine  N-acyltransferase (ceramide synthase) [  12].	transcription
59703	3	335977	5	NULL	NULL	0	NULL	ceramide synthase	GP		is					sphinganine N-acyltransferase	GP				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_177_1_109_s_11	10436928	Fumonisin is structurally related to sphingosine, and FB1 is a competitive inhibitor of sphinganine  N-acyltransferase (ceramide synthase) [  12].	transcription
78953	1	335977	6	NULL	NULL	0	NULL	Fumonisin	Chemical		is related to		structurally			sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_177_1_109_s_11	10436928	Fumonisin is structurally related to sphingosine, and FB1 is a competitive inhibitor of sphinganine  N-acyltransferase (ceramide synthase) [  12].	transcription
78954	2	335977	6	NULL	NULL	0	NULL	FB1	Chemical		is an inhibitor for		competitive			sphinganine N-acyltransferase	GP				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_177_1_109_s_11	10436928	Fumonisin is structurally related to sphingosine, and FB1 is a competitive inhibitor of sphinganine  N-acyltransferase (ceramide synthase) [  12].	transcription
78955	3	335977	6	NULL	NULL	0	NULL	sphinganine N-acyltransferase	GP		is					ceramide synthase	GP				NULL		0	NULL	NULL	NULL	gw60_femsmicrobiollett_177_1_109_s_11	10436928	Fumonisin is structurally related to sphingosine, and FB1 is a competitive inhibitor of sphinganine  N-acyltransferase (ceramide synthase) [  12].	transcription
59698	1	335978	5	NULL	NULL	0	NULL	sphingosine	Chemical		acylated to					PAP1	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_188_s_52	12531553	Schematic representation of the inhibition of the acylation of sphingosine by AP1, which is acylated to PAP1, a more potent inhibitor of ceramide synthase.	transcription
59699	2	335978	5	NULL	NULL	0	NULL	AP1	GP		catalyzes					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_188_s_52	12531553	Schematic representation of the inhibition of the acylation of sphingosine by AP1, which is acylated to PAP1, a more potent inhibitor of ceramide synthase.	transcription
59700	3	335978	5	NULL	NULL	0	NULL	PAP1	Chemical		is an inhibitor of		potent			ceramide synthase					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_188_s_52	12531553	Schematic representation of the inhibition of the acylation of sphingosine by AP1, which is acylated to PAP1, a more potent inhibitor of ceramide synthase.	transcription
78950	1	335978	6	NULL	NULL	0	NULL	AP1	GP		acylates					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_188_s_52	12531553	Schematic representation of the inhibition of the acylation of sphingosine by AP1, which is acylated to PAP1, a more potent inhibitor of ceramide synthase.	transcription
78951	2	335978	6	NULL	NULL	0	NULL	sphingosine	Chemical		is acylated into					PAP1	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_188_s_52	12531553	Schematic representation of the inhibition of the acylation of sphingosine by AP1, which is acylated to PAP1, a more potent inhibitor of ceramide synthase.	transcription
78952	3	335978	6	NULL	NULL	0	NULL	PAP1	GP		is an inhibitor for					ceramide synthase	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_188_s_52	12531553	Schematic representation of the inhibition of the acylation of sphingosine by AP1, which is acylated to PAP1, a more potent inhibitor of ceramide synthase.	transcription
59693	1	335979	5	NULL	NULL	0	NULL	LH	GP		induce					progesterone	GP	production of			NULL	hen granulosa cells	NULL	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_160	9915989	The effect of ceramide analogues and sphingosine on basal and LH-induced progesterone production in hen granulosa cells during follicular development.	transcription
59694	2	335979	5	NULL	NULL	0	NULL	ceramide analogues	Chemical		effects		potentially			statement 1					NULL	hen granulosa cells 	NULL	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_160	9915989	The effect of ceramide analogues and sphingosine on basal and LH-induced progesterone production in hen granulosa cells during follicular development.	transcription
59695	3	335979	5	NULL	NULL	0	NULL	statement 2	Process		occurs during					follicle	CellComponent	development of			NULL	hen granulosa cells 	NULL	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_160	9915989	The effect of ceramide analogues and sphingosine on basal and LH-induced progesterone production in hen granulosa cells during follicular development.	transcription
59696	4	335979	5	NULL	NULL	0	NULL	sphingosine	Chemical		effects		potentially			statement 1	Process				NULL	hen granulosa cells 	0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_160	9915989	The effect of ceramide analogues and sphingosine on basal and LH-induced progesterone production in hen granulosa cells during follicular development.	transcription
59697	5	335979	5	NULL	NULL	0	NULL	statement 4	Process		occurs during					follicle	CellComponent	development of			NULL	hen granulosa cells 	0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_160	9915989	The effect of ceramide analogues and sphingosine on basal and LH-induced progesterone production in hen granulosa cells during follicular development.	transcription
59686	1	335980	5	NULL	NULL	0	NULL	CDase	GP		is					ceramidase	GP				NULL		NULL	NULL	NULL	NULL	gw60_clindiagnlabimmun_6_1_101_s_11	9874672	Ceramidase (CDase), which catalyzes the cleavage of ceramide to fatty acids and sphingosine, is a known inhibitor of the protein kinase C.	transcription
59687	2	335980	5	NULL	NULL	0	NULL	ceramide	Chemical		is cleaved into					fatty acid	Chemical				NULL		0	NULL	NULL	NULL	gw60_clindiagnlabimmun_6_1_101_s_11	9874672	Ceramidase (CDase), which catalyzes the cleavage of ceramide to fatty acids and sphingosine, is a known inhibitor of the protein kinase C.	transcription
59688	3	335980	5	NULL	NULL	0	NULL	ceramide	Chemical		is cleaved into					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_clindiagnlabimmun_6_1_101_s_11	9874672	Ceramidase (CDase), which catalyzes the cleavage of ceramide to fatty acids and sphingosine, is a known inhibitor of the protein kinase C.	transcription
59689	4	335980	5	NULL	NULL	0	NULL	statement 2	Process		occurs along with					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_clindiagnlabimmun_6_1_101_s_11	9874672	Ceramidase (CDase), which catalyzes the cleavage of ceramide to fatty acids and sphingosine, is a known inhibitor of the protein kinase C.	transcription
59690	5	335980	5	NULL	NULL	0	NULL	CDase	GP		catalyzes					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_clindiagnlabimmun_6_1_101_s_11	9874672	Ceramidase (CDase), which catalyzes the cleavage of ceramide to fatty acids and sphingosine, is a known inhibitor of the protein kinase C.	transcription
59691	6	335980	5	NULL	NULL	0	NULL	CDase	GP		catalyzes					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_clindiagnlabimmun_6_1_101_s_11	9874672	Ceramidase (CDase), which catalyzes the cleavage of ceramide to fatty acids and sphingosine, is a known inhibitor of the protein kinase C.	transcription
59692	7	335980	5	NULL	NULL	0	NULL	CDase	GP		is an inhibitor of					protein kinase C	GP				NULL		0	NULL	NULL	NULL	gw60_clindiagnlabimmun_6_1_101_s_11	9874672	Ceramidase (CDase), which catalyzes the cleavage of ceramide to fatty acids and sphingosine, is a known inhibitor of the protein kinase C.	transcription
78944	1	335980	6	NULL	NULL	0	NULL	ceramide	Chemical		is cleaved to					fatty acids	Chemical				NULL		0	NULL	NULL	NULL	gw60_clindiagnlabimmun_6_1_101_s_11	9874672	Ceramidase (CDase), which catalyzes the cleavage of ceramide to fatty acids and sphingosine, is a known inhibitor of the protein kinase C.	transcription
78945	2	335980	6	NULL	NULL	0	NULL	ceramide	Chemical		is cleaved to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_clindiagnlabimmun_6_1_101_s_11	9874672	Ceramidase (CDase), which catalyzes the cleavage of ceramide to fatty acids and sphingosine, is a known inhibitor of the protein kinase C.	transcription
78946	3	335980	6	NULL	NULL	0	NULL	statement 1	Process		occurs simultaneously with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_clindiagnlabimmun_6_1_101_s_11	9874672	Ceramidase (CDase), which catalyzes the cleavage of ceramide to fatty acids and sphingosine, is a known inhibitor of the protein kinase C.	transcription
78947	4	335980	6	NULL	NULL	0	NULL	Ceramidase	GP		catalyzes					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_clindiagnlabimmun_6_1_101_s_11	9874672	Ceramidase (CDase), which catalyzes the cleavage of ceramide to fatty acids and sphingosine, is a known inhibitor of the protein kinase C.	transcription
78948	5	335980	6	NULL	NULL	0	NULL	Ceramidase	GP		is					CDase	GP				NULL		0	NULL	NULL	NULL	gw60_clindiagnlabimmun_6_1_101_s_11	9874672	Ceramidase (CDase), which catalyzes the cleavage of ceramide to fatty acids and sphingosine, is a known inhibitor of the protein kinase C.	transcription
78949	6	335980	6	NULL	NULL	0	NULL	CDase	GP		is an inhibitor for					protein kinase C	GP				NULL		0	NULL	NULL	NULL	gw60_clindiagnlabimmun_6_1_101_s_11	9874672	Ceramidase (CDase), which catalyzes the cleavage of ceramide to fatty acids and sphingosine, is a known inhibitor of the protein kinase C.	transcription
59707	1	335981	5	NULL	NULL	0	NULL	ceramide	Chemical		induce					apoptosis	Process				NULL	U937 cells	0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_28	9415703	The current study was undertaken to compare the relative involvement of SAPK activities in the induction of apoptosis by ceramide and sphingosine in U937 cells.	transcription
59708	2	335981	5	NULL	NULL	0	NULL	sphingosine	Chemical		induce					apoptosis	Process				NULL	U937 cells	NULL	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_28	9415703	The current study was undertaken to compare the relative involvement of SAPK activities in the induction of apoptosis by ceramide and sphingosine in U937 cells.	transcription
59709	3	335981	5	NULL	NULL	0	NULL	SAPK	GP	activity of	is involved in					statement 1	Process				NULL	U937 cells	NULL	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_28	9415703	The current study was undertaken to compare the relative involvement of SAPK activities in the induction of apoptosis by ceramide and sphingosine in U937 cells.	transcription
59710	4	335981	5	NULL	NULL	0	NULL	SAPK	GP	activity of	is involved in					statement 2	Process				NULL	U937 cells	NULL	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_28	9415703	The current study was undertaken to compare the relative involvement of SAPK activities in the induction of apoptosis by ceramide and sphingosine in U937 cells.	transcription
78942	1	335981	6	NULL	NULL	0	NULL	ceramide	Chemical		induces					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_28	9415703	The current study was undertaken to compare the relative involvement of SAPK activities in the induction of apoptosis by ceramide and sphingosine in U937 cells.	transcription
78943	2	335981	6	NULL	NULL	0	NULL	sphingosine	GP		induces					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_28	9415703	The current study was undertaken to compare the relative involvement of SAPK activities in the induction of apoptosis by ceramide and sphingosine in U937 cells.	transcription
59711	1	335982	5	NULL	NULL	0	NULL	ceramide	Chemical		induce					cell death	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_298	9415703	Increased expression and activation of the SAPK substrate c-Jun were absolutely necessary for the induction of cell death by ceramide but not by sphingosine.	transcription
59712	2	335982	5	NULL	NULL	0	NULL	c-Jun	GP		is a substrate of					SAPK	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_298	9415703	Increased expression and activation of the SAPK substrate c-Jun were absolutely necessary for the induction of cell death by ceramide but not by sphingosine.	transcription
59713	3	335982	5	NULL	NULL	0	NULL	c-Jun	GP	increased expression;;activation of	is necessary for					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_298	9415703	Increased expression and activation of the SAPK substrate c-Jun were absolutely necessary for the induction of cell death by ceramide but not by sphingosine.	transcription
59714	4	335982	5	NULL	NULL	0	NULL	sphingosine	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_298	9415703	Increased expression and activation of the SAPK substrate c-Jun were absolutely necessary for the induction of cell death by ceramide but not by sphingosine.	transcription
59715	5	335982	5	NULL	NULL	0	NULL	c-Jun	GP	increased expression;;activation of	is not necessary for					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_298	9415703	Increased expression and activation of the SAPK substrate c-Jun were absolutely necessary for the induction of cell death by ceramide but not by sphingosine.	transcription
78939	1	335982	6	NULL	NULL	0	NULL	ceramide	Chemical		induces					cell death	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_298	9415703	Increased expression and activation of the SAPK substrate c-Jun were absolutely necessary for the induction of cell death by ceramide but not by sphingosine.	transcription
78940	2	335982	6	NULL	NULL	0	NULL	c-jun	GP	activation of	is necessary for					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_298	9415703	Increased expression and activation of the SAPK substrate c-Jun were absolutely necessary for the induction of cell death by ceramide but not by sphingosine.	transcription
78941	3	335982	6	NULL	NULL	0	NULL	c-jun	GP	expression of	is necessary for					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_298	9415703	Increased expression and activation of the SAPK substrate c-Jun were absolutely necessary for the induction of cell death by ceramide but not by sphingosine.	transcription
59716	1	335983	5	NULL	NULL	0	NULL	N, N-dimethylsphingosine	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12724_s_371	11821388	Similarly, in the study of Sweeney  et al. ( 28),  N, N-dimethylsphingosine and sphingosine induced apoptosis in the absence of ceramide generation.	transcription
59717	2	335983	5	NULL	NULL	0	NULL	statement 1	Process		in the absence of					ceramide	Chemical	generation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12724_s_371	11821388	Similarly, in the study of Sweeney  et al. ( 28),  N, N-dimethylsphingosine and sphingosine induced apoptosis in the absence of ceramide generation.	transcription
59718	3	335983	5	NULL	NULL	0	NULL	sphingosine	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12724_s_371	11821388	Similarly, in the study of Sweeney  et al. ( 28),  N, N-dimethylsphingosine and sphingosine induced apoptosis in the absence of ceramide generation.	transcription
59719	4	335983	5	NULL	NULL	0	NULL	statement 3	Process		in the absence of					ceramide	Chemical	generation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12724_s_371	11821388	Similarly, in the study of Sweeney  et al. ( 28),  N, N-dimethylsphingosine and sphingosine induced apoptosis in the absence of ceramide generation.	transcription
78935	1	335983	6	NULL	NULL	0	NULL	N, N-dimethylsphingosine	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12724_s_371	11821388	Similarly, in the study of Sweeney  et al. ( 28),  N, N-dimethylsphingosine and sphingosine induced apoptosis in the absence of ceramide generation.	transcription
78936	2	335983	6	NULL	NULL	0	NULL	sphingosine	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12724_s_371	11821388	Similarly, in the study of Sweeney  et al. ( 28),  N, N-dimethylsphingosine and sphingosine induced apoptosis in the absence of ceramide generation.	transcription
78937	3	335983	6	NULL	NULL	0	NULL	statement 1	Process		occurs in absence of					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12724_s_371	11821388	Similarly, in the study of Sweeney  et al. ( 28),  N, N-dimethylsphingosine and sphingosine induced apoptosis in the absence of ceramide generation.	transcription
78938	4	335983	6	NULL	NULL	0	NULL	statement 2	Process		occurs in absence of					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12724_s_371	11821388	Similarly, in the study of Sweeney  et al. ( 28),  N, N-dimethylsphingosine and sphingosine induced apoptosis in the absence of ceramide generation.	transcription
59720	1	335984	5	NULL	NULL	0	NULL	ceramide	Chemical		induce					cell death	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_27129_s_121	11369765	These results indicated that ceramide and sphingosine can induce cell death regardless of the presence or absence of p53.	transcription
59721	2	335984	5	NULL	NULL	0	NULL	sphingosine	Chemical		induce					cell death	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_27129_s_121	11369765	These results indicated that ceramide and sphingosine can induce cell death regardless of the presence or absence of p53.	transcription
78933	1	335984	6	NULL	NULL	0	NULL	ceramide	Chemical		induce					cell death	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_27129_s_121	11369765	These results indicated that ceramide and sphingosine can induce cell death regardless of the presence or absence of p53.	transcription
78934	2	335984	6	NULL	NULL	0	NULL	sphingosine	Chemical		induce					cell death	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_29_27129_s_121	11369765	These results indicated that ceramide and sphingosine can induce cell death regardless of the presence or absence of p53.	transcription
59722	1	335985	5	NULL	NULL	0	NULL	Fas	GP		induce					ceramide	Chemical	generation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_62	10747891	Fas induces generation of ceramide and sphingosine prior to activation of caspases and formation of apoptotic nuclei.	transcription
59723	2	335985	5	NULL	NULL	0	NULL	Fas	GP		induce					sphingosine	Chemical	generation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_62	10747891	Fas induces generation of ceramide and sphingosine prior to activation of caspases and formation of apoptotic nuclei.	transcription
59724	3	335985	5	NULL	NULL	0	NULL	statement 1	Process		occurs prior to					caspases	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_62	10747891	Fas induces generation of ceramide and sphingosine prior to activation of caspases and formation of apoptotic nuclei.	transcription
59725	4	335985	5	NULL	NULL	0	NULL	statement 1	Process		occurs prior to					apoptotic nuclei	CellComponent	formation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_62	10747891	Fas induces generation of ceramide and sphingosine prior to activation of caspases and formation of apoptotic nuclei.	transcription
59726	5	335985	5	NULL	NULL	0	NULL	statement 2	Process		occurs prior to					caspases	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_62	10747891	Fas induces generation of ceramide and sphingosine prior to activation of caspases and formation of apoptotic nuclei.	transcription
59727	6	335985	5	NULL	NULL	0	NULL	statement 2	Process		occurs prior to					apoptotic nuclei	CellComponent	formation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_62	10747891	Fas induces generation of ceramide and sphingosine prior to activation of caspases and formation of apoptotic nuclei.	transcription
78927	1	335985	6	NULL	NULL	0	NULL	Fas	GP		induces					ceramide	Chemical	generation of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_62	10747891	Fas induces generation of ceramide and sphingosine prior to activation of caspases and formation of apoptotic nuclei.	transcription
78928	2	335985	6	NULL	NULL	0	NULL	Fas	GP		induces					sphingosine	Chemical	generation of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_62	10747891	Fas induces generation of ceramide and sphingosine prior to activation of caspases and formation of apoptotic nuclei.	transcription
78929	3	335985	6	NULL	NULL	0	NULL	statement 1	Process		occurs prior to					caspases	GP	activation of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_62	10747891	Fas induces generation of ceramide and sphingosine prior to activation of caspases and formation of apoptotic nuclei.	transcription
78930	4	335985	6	NULL	NULL	0	NULL	statement 2	Process		occurs prior to					caspases	GP	activation of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_62	10747891	Fas induces generation of ceramide and sphingosine prior to activation of caspases and formation of apoptotic nuclei.	transcription
78931	5	335985	6	NULL	NULL	0	NULL	statement 1	Process		occurs prior to					apoptotic nuclei	CellComponent	formation of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_62	10747891	Fas induces generation of ceramide and sphingosine prior to activation of caspases and formation of apoptotic nuclei.	transcription
78932	6	335985	6	NULL	NULL	0	NULL	statement 2	Process		occurs prior to					apoptotic nuclei	CellComponent	formation of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_62	10747891	Fas induces generation of ceramide and sphingosine prior to activation of caspases and formation of apoptotic nuclei.	transcription
59728	1	335986	5	NULL	NULL	0	NULL	sphingosine	Chemical	increase in;;generation of	is triggerd by					Fas	GP	ligation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_130	10747891	In agreement, we found that overexpression of Bcl-xL did not inhibit the early increase in ceramide or sphingosine generation triggered by Fas ligation.	transcription
59729	2	335986	5	NULL	NULL	0	NULL	ceramide	Chemical	increase in;;generation of	is triggerd by					Fas	GP	ligation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_130	10747891	In agreement, we found that overexpression of Bcl-xL did not inhibit the early increase in ceramide or sphingosine generation triggered by Fas ligation.	transcription
59730	3	335986	5	NULL	NULL	0	NULL	Bcl-xL	GP	overexpression of	does not inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_130	10747891	In agreement, we found that overexpression of Bcl-xL did not inhibit the early increase in ceramide or sphingosine generation triggered by Fas ligation.	transcription
59731	4	335986	5	NULL	NULL	0	NULL	Bcl-xL	GP	overexpression of	does not inhibit					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_130	10747891	In agreement, we found that overexpression of Bcl-xL did not inhibit the early increase in ceramide or sphingosine generation triggered by Fas ligation.	transcription
59732	1	335987	5	NULL	NULL	0	NULL	cyt c	GP		is translocated from					mitochondria	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_183	10747891	These results demonstrate that sphingosine and ceramide induce translocation of cyt  c from mitochondria to cytosol in a caspase-independent manner.	transcription
59733	2	335987	5	NULL	NULL	0	NULL	cyt c	GP		is translocated to					cytosol	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_183	10747891	These results demonstrate that sphingosine and ceramide induce translocation of cyt  c from mitochondria to cytosol in a caspase-independent manner.	transcription
59734	3	335987	5	NULL	NULL	0	NULL	statement 1	Process		occurs along with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_183	10747891	These results demonstrate that sphingosine and ceramide induce translocation of cyt  c from mitochondria to cytosol in a caspase-independent manner.	transcription
59735	4	335987	5	NULL	NULL	0	NULL	sphingosine	Chemical		induce					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_183	10747891	These results demonstrate that sphingosine and ceramide induce translocation of cyt  c from mitochondria to cytosol in a caspase-independent manner.	transcription
59736	5	335987	5	NULL	NULL	0	NULL	statement 4	Process		is independent of					caspase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_183	10747891	These results demonstrate that sphingosine and ceramide induce translocation of cyt  c from mitochondria to cytosol in a caspase-independent manner.	transcription
59737	6	335987	5	NULL	NULL	0	NULL	ceramide	Chemical		induce					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_183	10747891	These results demonstrate that sphingosine and ceramide induce translocation of cyt  c from mitochondria to cytosol in a caspase-independent manner.	transcription
59738	7	335987	5	NULL	NULL	0	NULL	statement 6	Process		is independent of					caspase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_183	10747891	These results demonstrate that sphingosine and ceramide induce translocation of cyt  c from mitochondria to cytosol in a caspase-independent manner.	transcription
78922	1	335987	6	NULL	NULL	0	NULL	cyt c	GP		is translocated from					mitochondria	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_183	10747891	These results demonstrate that sphingosine and ceramide induce translocation of cyt  c from mitochondria to cytosol in a caspase-independent manner.	transcription
78923	2	335987	6	NULL	NULL	0	NULL	cyt c	GP		is translocated to					cytosol	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_183	10747891	These results demonstrate that sphingosine and ceramide induce translocation of cyt  c from mitochondria to cytosol in a caspase-independent manner.	transcription
78924	3	335987	6	NULL	NULL	0	NULL	statement 1	Process		occurs simultaneously with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_183	10747891	These results demonstrate that sphingosine and ceramide induce translocation of cyt  c from mitochondria to cytosol in a caspase-independent manner.	transcription
78925	4	335987	6	NULL	NULL	0	NULL	sphingosine	Chemical		induces					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_183	10747891	These results demonstrate that sphingosine and ceramide induce translocation of cyt  c from mitochondria to cytosol in a caspase-independent manner.	transcription
78926	5	335987	6	NULL	NULL	0	NULL	ceramide	Chemical		induces					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_183	10747891	These results demonstrate that sphingosine and ceramide induce translocation of cyt  c from mitochondria to cytosol in a caspase-independent manner.	transcription
59739	1	335988	5	NULL	NULL	0	NULL	ceramide	Chemical	formation of	is mediated by					cytokine	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_48_37365_s_246	10956644	B, cytokine-mediated formation of [3]ceramide and [3]sphingosine from the newly delivered [3]sphingomyelin.	transcription
59740	2	335988	5	NULL	NULL	0	NULL	sphingosine	Chemical	formation of	is mediated by					cytokine	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_48_37365_s_246	10956644	B, cytokine-mediated formation of [3]ceramide and [3]sphingosine from the newly delivered [3]sphingomyelin.	transcription
59741	3	335988	5	NULL	NULL	0	NULL	ceramide	Chemical		is formed from					sphingomyelin	Chemical	newly delivered			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_48_37365_s_246	10956644	B, cytokine-mediated formation of [3]ceramide and [3]sphingosine from the newly delivered [3]sphingomyelin.	transcription
59742	4	335988	5	NULL	NULL	0	NULL	sphingosine	Chemical		is formed from					sphingomyelin	Chemical	newly delivered			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_48_37365_s_246	10956644	B, cytokine-mediated formation of [3]ceramide and [3]sphingosine from the newly delivered [3]sphingomyelin.	transcription
78920	1	335988	6	NULL	NULL	0	NULL	sphingomyelin	Chemical		forms					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_48_37365_s_246	10956644	B, cytokine-mediated formation of [3]ceramide and [3]sphingosine from the newly delivered [3]sphingomyelin.	transcription
78921	2	335988	6	NULL	NULL	0	NULL	sphingomyelin	Chemical		forms					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_48_37365_s_246	10956644	B, cytokine-mediated formation of [3]ceramide and [3]sphingosine from the newly delivered [3]sphingomyelin.	transcription
59743	1	335989	5	NULL	NULL	0	NULL	apoptosis	Process		is induced by					ceramide	Chemical				NULL	U937 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_182	8626522	Ceramide-induced apoptosis was comparably enhanced by sphingosine and  sphinganine in U937 cells (data not shown).	transcription
59744	2	335989	5	NULL	NULL	0	NULL	sphingosine	Chemical		enhances					statement 1	Process				NULL	U937 cells	0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_182	8626522	Ceramide-induced apoptosis was comparably enhanced by sphingosine and  sphinganine in U937 cells (data not shown).	transcription
59745	3	335989	5	NULL	NULL	0	NULL	sphinganine	Chemical		enhances					statement 1	Process				NULL	U937 cells	0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_182	8626522	Ceramide-induced apoptosis was comparably enhanced by sphingosine and  sphinganine in U937 cells (data not shown).	transcription
78917	1	335989	6	NULL	NULL	0	NULL	ceramide	Chemical		induces					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_182	8626522	Ceramide-induced apoptosis was comparably enhanced by sphingosine and  sphinganine in U937 cells (data not shown).	transcription
78918	2	335989	6	NULL	NULL	0	NULL	sphingosine	Chemical		enhances					statement 1	Process				NULL	U937 cells	0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_182	8626522	Ceramide-induced apoptosis was comparably enhanced by sphingosine and  sphinganine in U937 cells (data not shown).	transcription
78919	3	335989	6	NULL	NULL	NULL	NULL	sphinganine	Chemical		enhances					statement 1	Process				NULL	U937 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_182	8626522	Ceramide-induced apoptosis was comparably enhanced by sphingosine and  sphinganine in U937 cells (data not shown).	transcription
59746	1	335991	5	NULL	NULL	0	NULL	phospholipase D	GP		is activated by					sphingosine 1-phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_8	7592842	Okadaic acid decreased the activation of phospholipase D by  sphingosine 1-phosphate and did not reverse the inhibitory effect of  C -ceramide on this activation.	transcription
59747	2	335991	5	NULL	NULL	0	NULL	okadaic acid	Chemical		decreases					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_8	7592842	Okadaic acid decreased the activation of phospholipase D by  sphingosine 1-phosphate and did not reverse the inhibitory effect of  C -ceramide on this activation.	transcription
59748	3	335991	5	NULL	NULL	0	NULL	C -ceramide	Chemical		inhibits					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_8	7592842	Okadaic acid decreased the activation of phospholipase D by  sphingosine 1-phosphate and did not reverse the inhibitory effect of  C -ceramide on this activation.	transcription
59749	4	335991	5	NULL	NULL	0	NULL	okadaic acid	Chemical		does not reverse					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_8	7592842	Okadaic acid decreased the activation of phospholipase D by  sphingosine 1-phosphate and did not reverse the inhibitory effect of  C -ceramide on this activation.	transcription
78915	1	335991	6	NULL	NULL	NULL	NULL	Okadaic acid	Chemical		decreases					phospholipase D	GP	activation of 			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_8	7592842	Okadaic acid decreased the activation of phospholipase D by  sphingosine 1-phosphate and did not reverse the inhibitory effect of  C -ceramide on this activation.	transcription
78916	2	335991	6	NULL	NULL	0	NULL	statement 1	Process		occurs via					sphingosine 1-phosphate	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_8	7592842	Okadaic acid decreased the activation of phospholipase D by  sphingosine 1-phosphate and did not reverse the inhibitory effect of  C -ceramide on this activation.	transcription
59750	1	335992	5	NULL	NULL	0	NULL	cAMP	Chemical		is produced by					SPP	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_171	7592842	However, there was no significant effect of  C -ceramide on the percentage decrease in cAMP that was  produced by SPP, sphingosine, and lysophosphatidate ( Table 1).	transcription
59751	2	335992	5	NULL	NULL	0	NULL	cAMP	Chemical		is produced by					sphingosine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_171	7592842	However, there was no significant effect of  C -ceramide on the percentage decrease in cAMP that was  produced by SPP, sphingosine, and lysophosphatidate ( Table 1).	transcription
59752	3	335992	5	NULL	NULL	0	NULL	cAMP	Chemical		is produced by					lysophosphatidate	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_171	7592842	However, there was no significant effect of  C -ceramide on the percentage decrease in cAMP that was  produced by SPP, sphingosine, and lysophosphatidate ( Table 1).	transcription
59753	4	335992	5	NULL	NULL	0	NULL	C -ceramide	Chemical		does not effect		significantly			statement 1	Process	decrease in			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_171	7592842	However, there was no significant effect of  C -ceramide on the percentage decrease in cAMP that was  produced by SPP, sphingosine, and lysophosphatidate ( Table 1).	transcription
59754	5	335992	5	NULL	NULL	0	NULL	C -ceramide	Chemical		does not effect		significantly			statement 2	Process	decrease in			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_171	7592842	However, there was no significant effect of  C -ceramide on the percentage decrease in cAMP that was  produced by SPP, sphingosine, and lysophosphatidate ( Table 1).	transcription
59755	6	335992	5	NULL	NULL	0	NULL	C -ceramide	Chemical		does not effect		significantly			statement 3	Process	decrease in			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_171	7592842	However, there was no significant effect of  C -ceramide on the percentage decrease in cAMP that was  produced by SPP, sphingosine, and lysophosphatidate ( Table 1).	transcription
78912	1	335992	6	NULL	NULL	0	NULL	SPP	Chemical		produces					cAMP	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_171	7592842	However, there was no significant effect of  C -ceramide on the percentage decrease in cAMP that was  produced by SPP, sphingosine, and lysophosphatidate ( Table 1).	transcription
78913	2	335992	6	NULL	NULL	0	NULL	sphingosine	Chemical		produces					cAMP	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_171	7592842	However, there was no significant effect of  C -ceramide on the percentage decrease in cAMP that was  produced by SPP, sphingosine, and lysophosphatidate ( Table 1).	transcription
78914	3	335992	6	NULL	NULL	0	NULL	lysophosphatidate	Chemical		produces					cAMP	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_171	7592842	However, there was no significant effect of  C -ceramide on the percentage decrease in cAMP that was  produced by SPP, sphingosine, and lysophosphatidate ( Table 1).	transcription
59756	1	335993	5	NULL	NULL	0	NULL	sphingosine	Chemical		induce					apoptosis	Process				NULL	in cells in culture 	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_48_33875_s_177	10567348	If so, the formation of sphingosine and ceramide, which are well known to induce apoptosis in cells in culture ( 1-4), might participate in the toxicity of NH4+.	transcription
59757	2	335993	5	NULL	NULL	0	NULL	ceramide	Chemical		induce					apoptosis	Process				NULL	in cells in culture	0	NULL	NULL	NULL	gw60_jbiolchem_274_48_33875_s_177	10567348	If so, the formation of sphingosine and ceramide, which are well known to induce apoptosis in cells in culture ( 1-4), might participate in the toxicity of NH4+.	transcription
59758	3	335993	5	NULL	NULL	0	NULL	sphingosine	Chemical	formation of	participates in		might			NH4+	Chemical	toxicity of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_48_33875_s_177	10567348	If so, the formation of sphingosine and ceramide, which are well known to induce apoptosis in cells in culture ( 1-4), might participate in the toxicity of NH4+.	transcription
59759	4	335993	5	NULL	NULL	0	NULL	ceramide	Chemical	formation of	participates in		might			NH4+	Chemical	toxicity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_48_33875_s_177	10567348	If so, the formation of sphingosine and ceramide, which are well known to induce apoptosis in cells in culture ( 1-4), might participate in the toxicity of NH4+.	transcription
78910	1	335993	6	NULL	NULL	0	NULL	sphingosine	Chemical		induces					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_48_33875_s_177	10567348	If so, the formation of sphingosine and ceramide, which are well known to induce apoptosis in cells in culture ( 1-4), might participate in the toxicity of NH4+.	transcription
78911	2	335993	6	NULL	NULL	0	NULL	ceramide	Chemical		induces					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_48_33875_s_177	10567348	If so, the formation of sphingosine and ceramide, which are well known to induce apoptosis in cells in culture ( 1-4), might participate in the toxicity of NH4+.	transcription
59760	1	335994	5	NULL	NULL	0	NULL	TNF-alpha	g		increases					ceramide	Chemical	cellular concentration of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_25_15345_s_194	9624115	TNF-alpha increased the cellular concentration of ceramide, but TNF-alpha had no effect on the amount of basal sphingosine.	transcription
59761	2	335994	5	NULL	NULL	0	NULL	TNF-alpha	GP		does not effect					sphingosine	Chemical	basal amount of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_25_15345_s_194	9624115	TNF-alpha increased the cellular concentration of ceramide, but TNF-alpha had no effect on the amount of basal sphingosine.	transcription
78908	1	335994	6	NULL	NULL	0	NULL	TNF-alpha	Chemical		increases					ceramide	Chemical	levels of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_25_15345_s_194	9624115	TNF-alpha increased the cellular concentration of ceramide, but TNF-alpha had no effect on the amount of basal sphingosine.	transcription
78909	2	335994	6	NULL	NULL	0	NULL	TNF-alpha	GP		has no effect on					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_25_15345_s_194	9624115	TNF-alpha increased the cellular concentration of ceramide, but TNF-alpha had no effect on the amount of basal sphingosine.	transcription
59762	1	335995	5	NULL	NULL	0	NULL	PMA	Chemical		increases					sphingosine	Chemical	level of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_25_15345_s_196	9624115	In contrast to TNF-alpha, PMA increased sphingosine levels but did not increase basal levels of ceramide, even in the presence of TNF-alpha.	transcription
59763	2	335995	5	NULL	NULL	0	NULL	PMA	Chemical		does not increase					ceramide	Chemical	basal level of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_25_15345_s_196	9624115	In contrast to TNF-alpha, PMA increased sphingosine levels but did not increase basal levels of ceramide, even in the presence of TNF-alpha.	transcription
59764	3	335995	5	NULL	NULL	0	NULL	statement 2	Process		in the presence of					TNF-alpha	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_25_15345_s_196	9624115	In contrast to TNF-alpha, PMA increased sphingosine levels but did not increase basal levels of ceramide, even in the presence of TNF-alpha.	transcription
78906	1	335995	6	NULL	NULL	0	NULL	PMA	Chemical		increases					sphingosine	Chemical	levels of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_25_15345_s_196	9624115	In contrast to TNF-alpha, PMA increased sphingosine levels but did not increase basal levels of ceramide, even in the presence of TNF-alpha.	transcription
78907	2	335995	6	NULL	NULL	0	NULL	PMA	Chemical		does not increase					ceramide	Chemical	levels of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_25_15345_s_196	9624115	In contrast to TNF-alpha, PMA increased sphingosine levels but did not increase basal levels of ceramide, even in the presence of TNF-alpha.	transcription
59765	1	335996	5	NULL	NULL	0	NULL	LPP1 gene product	GP	PA phosphatase activity of	is independent of					Mg2+	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_23_14331_s_170	9603941	We examined the effects of ceramide 1-phosphate and sphingosine 1-phosphate on the Mg2+-independent PA phosphatase activity encoded by the  LPP1 gene.	transcription
59766	2	335996	5	NULL	NULL	0	NULL	ceramide 1-phosphate	Chemical		effects		potentially			statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_23_14331_s_170	9603941	We examined the effects of ceramide 1-phosphate and sphingosine 1-phosphate on the Mg2+-independent PA phosphatase activity encoded by the  LPP1 gene.	transcription
59767	3	335996	5	NULL	NULL	0	NULL	sphingosine 1-phosphate	Chemical		effects		potentially			statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_23_14331_s_170	9603941	We examined the effects of ceramide 1-phosphate and sphingosine 1-phosphate on the Mg2+-independent PA phosphatase activity encoded by the  LPP1 gene.	transcription
78904	1	335996	6	NULL	NULL	0	NULL	LPP1 gene	GP		encodes					PA phosphatase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_23_14331_s_170	9603941	We examined the effects of ceramide 1-phosphate and sphingosine 1-phosphate on the Mg2+-independent PA phosphatase activity encoded by the  LPP1 gene.	transcription
78905	2	335996	6	NULL	NULL	0	NULL	statement 1	Process		is independent of					Mg2+	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_23_14331_s_170	9603941	We examined the effects of ceramide 1-phosphate and sphingosine 1-phosphate on the Mg2+-independent PA phosphatase activity encoded by the  LPP1 gene.	transcription
59768	1	335997	5	NULL	NULL	0	NULL	PKC	GP		activates					sphingosine kinase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_17	9446602	These results indicate that PKC may inhibit ceramide-induced apoptosis by activating sphingosine kinase.	transcription
59769	2	335997	5	NULL	NULL	0	NULL	apoptosis	Process		is inhibited by					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_17	9446602	These results indicate that PKC may inhibit ceramide-induced apoptosis by activating sphingosine kinase.	transcription
59770	3	335997	5	NULL	NULL	0	NULL	statement 1	Process		inhibit		may			statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_17	9446602	These results indicate that PKC may inhibit ceramide-induced apoptosis by activating sphingosine kinase.	transcription
78900	1	335997	6	NULL	NULL	0	NULL	PKC	GP		activates					sphingosine kinase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_17	9446602	These results indicate that PKC may inhibit ceramide-induced apoptosis by activating sphingosine kinase.	transcription
78901	2	335997	6	NULL	NULL	0	NULL	ceramide	Chemical		induces					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_17	9446602	These results indicate that PKC may inhibit ceramide-induced apoptosis by activating sphingosine kinase.	transcription
78902	3	335997	6	NULL	NULL	0	NULL	PKC	GP		inhibits					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_17	9446602	These results indicate that PKC may inhibit ceramide-induced apoptosis by activating sphingosine kinase.	transcription
78903	4	335997	6	NULL	NULL	0	NULL	statement 3	Process		occurs via					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_17	9446602	These results indicate that PKC may inhibit ceramide-induced apoptosis by activating sphingosine kinase.	transcription
59771	1	335998	5	NULL	NULL	0	NULL	apoptosis	Process		is mediated by					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_1_1_s_107	9469581	Ceramide-mediated apoptosis is subject to reciprocal modulation by diglyceride and sphingosine in HL-60 and U937 human leukemia cells.	transcription
59772	2	335998	5	NULL	NULL	0	NULL	diglyceride	Chemical		modulate		reciprocally			statement 1	Process				NULL	HL-60 cells	0	NULL	NULL	NULL	gw60_jlipidres_39_1_1_s_107	9469581	Ceramide-mediated apoptosis is subject to reciprocal modulation by diglyceride and sphingosine in HL-60 and U937 human leukemia cells.	transcription
59773	3	335998	5	NULL	NULL	0	NULL	sphingosine	Chemical		modulate		reciprocally			statement 1	Process				NULL	HL-60 cells	0	NULL	NULL	NULL	gw60_jlipidres_39_1_1_s_107	9469581	Ceramide-mediated apoptosis is subject to reciprocal modulation by diglyceride and sphingosine in HL-60 and U937 human leukemia cells.	transcription
59774	6	335998	5	NULL	NULL	0	NULL	U937 cells	Cell		is a type of					human leukemia cells	Cell				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_1_1_s_107	9469581	Ceramide-mediated apoptosis is subject to reciprocal modulation by diglyceride and sphingosine in HL-60 and U937 human leukemia cells.	transcription
59775	4	335998	5	NULL	NULL	0	NULL	diglyceride	Chemical		modulate		reciprocally			statement 1	Process				NULL	U937 cells	NULL	NULL	NULL	NULL	gw60_jlipidres_39_1_1_s_107	9469581	Ceramide-mediated apoptosis is subject to reciprocal modulation by diglyceride and sphingosine in HL-60 and U937 human leukemia cells.	transcription
59776	5	335998	5	NULL	NULL	0	NULL	sphingosine	Chemical		modulate		reciprocally			statement 1	Process				NULL	U937 cells	NULL	NULL	NULL	NULL	gw60_jlipidres_39_1_1_s_107	9469581	Ceramide-mediated apoptosis is subject to reciprocal modulation by diglyceride and sphingosine in HL-60 and U937 human leukemia cells.	transcription
78899	1	335998	6	NULL	NULL	0	NULL	ceramide	Chemical		mediates					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_1_1_s_107	9469581	Ceramide-mediated apoptosis is subject to reciprocal modulation by diglyceride and sphingosine in HL-60 and U937 human leukemia cells.	transcription
59777	1	335999	5	NULL	NULL	0	NULL	DMS	Chemical		is					dimethylsphingosine	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_j-physiol_575_pt-1_16740613_s_8	16740613	This sensitizing action of NGF,  ceramide and internally perfused Sph was abolished by dimethylsphingosine  (DMS), an inhibitor of sphingosine kinase.	transcription
59778	2	335999	5	NULL	NULL	0	NULL	DMS	Chemical		is an inhibitor of					sphingosine kinase	GP				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_j-physiol_575_pt-1_16740613_s_8	16740613	This sensitizing action of NGF,  ceramide and internally perfused Sph was abolished by dimethylsphingosine  (DMS), an inhibitor of sphingosine kinase.	transcription
59779	3	335999	5	NULL	NULL	0	NULL	DMS	Chemical		abolishes					NGF	GP	sensitizing action of			NULL		0	NULL	NULL	NULL	abs-batch0740-0759_j-physiol_575_pt-1_16740613_s_8	16740613	This sensitizing action of NGF,  ceramide and internally perfused Sph was abolished by dimethylsphingosine  (DMS), an inhibitor of sphingosine kinase.	transcription
59780	4	335999	5	NULL	NULL	0	NULL	DMS	Chemical		abolishes					ceramide	Chemical	sensitizing action of			NULL		0	NULL	NULL	NULL	abs-batch0740-0759_j-physiol_575_pt-1_16740613_s_8	16740613	This sensitizing action of NGF,  ceramide and internally perfused Sph was abolished by dimethylsphingosine  (DMS), an inhibitor of sphingosine kinase.	transcription
59781	5	335999	5	NULL	NULL	0	NULL	DMS	Chemical		abolishes					Sph	Chemical	sensitizing action of;;internally perfused			NULL		0	NULL	NULL	NULL	abs-batch0740-0759_j-physiol_575_pt-1_16740613_s_8	16740613	This sensitizing action of NGF,  ceramide and internally perfused Sph was abolished by dimethylsphingosine  (DMS), an inhibitor of sphingosine kinase.	transcription
78897	1	335999	6	NULL	NULL	0	NULL	DMS	Chemical		is					dimethylsphingosine	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_j-physiol_575_pt-1_16740613_s_8	16740613	This sensitizing action of NGF,  ceramide and internally perfused Sph was abolished by dimethylsphingosine  (DMS), an inhibitor of sphingosine kinase.	transcription
78898	2	335999	6	NULL	NULL	0	NULL	DMS	Chemical		inhibits					sphingosine kinase	GP				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_j-physiol_575_pt-1_16740613_s_8	16740613	This sensitizing action of NGF,  ceramide and internally perfused Sph was abolished by dimethylsphingosine  (DMS), an inhibitor of sphingosine kinase.	transcription
59782	1	336000	5	NULL	NULL	0	NULL	sphingosine	Chemical		is phosphorylated to					SPP	Chemical				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_17	10760461	In contrast to the growth-inhibitory and pro-apoptotic effects of ceramide and sphingosine, SPP, which is produced by sphingosine kinase-dependent phosphorylation of sphingosine, has been implicated in cell growth [  8] and is able to inhibit ceramide-mediated apoptosis [  9,   10,   11 and   12].	transcription
59783	2	336000	5	NULL	NULL	0	NULL	statement 1	Process		is dependent on					sphingosine kinase	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_17	10760461	In contrast to the growth-inhibitory and pro-apoptotic effects of ceramide and sphingosine, SPP, which is produced by sphingosine kinase-dependent phosphorylation of sphingosine, has been implicated in cell growth [  8] and is able to inhibit ceramide-mediated apoptosis [  9,   10,   11 and   12].	transcription
59784	3	336000	5	NULL	NULL	0	NULL	SPP	Chemical		is implicated in					cell growth	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_17	10760461	In contrast to the growth-inhibitory and pro-apoptotic effects of ceramide and sphingosine, SPP, which is produced by sphingosine kinase-dependent phosphorylation of sphingosine, has been implicated in cell growth [  8] and is able to inhibit ceramide-mediated apoptosis [  9,   10,   11 and   12].	transcription
59785	4	336000	5	NULL	NULL	0	NULL	apoptosis	Process		is mediated by					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_17	10760461	In contrast to the growth-inhibitory and pro-apoptotic effects of ceramide and sphingosine, SPP, which is produced by sphingosine kinase-dependent phosphorylation of sphingosine, has been implicated in cell growth [  8] and is able to inhibit ceramide-mediated apoptosis [  9,   10,   11 and   12].	transcription
59786	5	336000	5	NULL	NULL	0	NULL	SPP	Chemical		inhibit					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_17	10760461	In contrast to the growth-inhibitory and pro-apoptotic effects of ceramide and sphingosine, SPP, which is produced by sphingosine kinase-dependent phosphorylation of sphingosine, has been implicated in cell growth [  8] and is able to inhibit ceramide-mediated apoptosis [  9,   10,   11 and   12].	transcription
78890	1	336000	6	NULL	NULL	0	NULL	ceramide	Chemical		inhibits					growth	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_17	10760461	In contrast to the growth-inhibitory and pro-apoptotic effects of ceramide and sphingosine, SPP, which is produced by sphingosine kinase-dependent phosphorylation of sphingosine, has been implicated in cell growth [  8] and is able to inhibit ceramide-mediated apoptosis [  9,   10,   11 and   12].	transcription
78891	2	336000	6	NULL	NULL	0	NULL	sphingosine	Chemical		inhibits					growth	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_17	10760461	In contrast to the growth-inhibitory and pro-apoptotic effects of ceramide and sphingosine, SPP, which is produced by sphingosine kinase-dependent phosphorylation of sphingosine, has been implicated in cell growth [  8] and is able to inhibit ceramide-mediated apoptosis [  9,   10,   11 and   12].	transcription
78892	3	336000	6	NULL	NULL	0	NULL	sphingosine	Chemical	phosphorylation of	is dependent on					sphingosine kinase	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_17	10760461	In contrast to the growth-inhibitory and pro-apoptotic effects of ceramide and sphingosine, SPP, which is produced by sphingosine kinase-dependent phosphorylation of sphingosine, has been implicated in cell growth [  8] and is able to inhibit ceramide-mediated apoptosis [  9,   10,   11 and   12].	transcription
78893	4	336000	6	NULL	NULL	0	NULL	statement 3	Process		produces					SPP	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_17	10760461	In contrast to the growth-inhibitory and pro-apoptotic effects of ceramide and sphingosine, SPP, which is produced by sphingosine kinase-dependent phosphorylation of sphingosine, has been implicated in cell growth [  8] and is able to inhibit ceramide-mediated apoptosis [  9,   10,   11 and   12].	transcription
78894	5	336000	6	NULL	NULL	0	NULL	SPP	GP		plays a role in					cell growth	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_17	10760461	In contrast to the growth-inhibitory and pro-apoptotic effects of ceramide and sphingosine, SPP, which is produced by sphingosine kinase-dependent phosphorylation of sphingosine, has been implicated in cell growth [  8] and is able to inhibit ceramide-mediated apoptosis [  9,   10,   11 and   12].	transcription
78895	6	336000	6	NULL	NULL	0	NULL	ceramide	Chemical		mediates					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_17	10760461	In contrast to the growth-inhibitory and pro-apoptotic effects of ceramide and sphingosine, SPP, which is produced by sphingosine kinase-dependent phosphorylation of sphingosine, has been implicated in cell growth [  8] and is able to inhibit ceramide-mediated apoptosis [  9,   10,   11 and   12].	transcription
78896	7	336000	6	NULL	NULL	0	NULL	SPP	Chemical		inhibits					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1484_2_107_s_17	10760461	In contrast to the growth-inhibitory and pro-apoptotic effects of ceramide and sphingosine, SPP, which is produced by sphingosine kinase-dependent phosphorylation of sphingosine, has been implicated in cell growth [  8] and is able to inhibit ceramide-mediated apoptosis [  9,   10,   11 and   12].	transcription
59787	1	336001	5	NULL	NULL	0	NULL	ceramide	Chemical	apoptotic capacity of	augmented by					D-erythro-sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_259	8626522	Thus, the findings that  the apoptotic capacity of ceramide was ( a) comparably  augmented by both D- and L- forms of  erythro-sphingosine and  threo-sphingosine, but ( b) selectively abolished by  sn-1,2-substituted (but  not  sn-2,3-substituted or  rac-1,3-substituted) forms  of diglyceride additionally supports an involvement of PKC activity in  the reciprocal modulation of ceramide action by sphingosine and  diglyceride.	transcription
59788	2	336001	5	NULL	NULL	0	NULL	ceramide	Chemical	apoptotic capacity of	augmented by					L-erythro-sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_259	8626522	Thus, the findings that  the apoptotic capacity of ceramide was ( a) comparably  augmented by both D- and L- forms of  erythro-sphingosine and  threo-sphingosine, but ( b) selectively abolished by  sn-1,2-substituted (but  not  sn-2,3-substituted or  rac-1,3-substituted) forms  of diglyceride additionally supports an involvement of PKC activity in  the reciprocal modulation of ceramide action by sphingosine and  diglyceride.	transcription
59789	3	336001	5	NULL	NULL	0	NULL	ceramide	Chemical	apoptotic capacity of	augmented by					threo-sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_259	8626522	Thus, the findings that  the apoptotic capacity of ceramide was ( a) comparably  augmented by both D- and L- forms of  erythro-sphingosine and  threo-sphingosine, but ( b) selectively abolished by  sn-1,2-substituted (but  not  sn-2,3-substituted or  rac-1,3-substituted) forms  of diglyceride additionally supports an involvement of PKC activity in  the reciprocal modulation of ceramide action by sphingosine and  diglyceride.	transcription
59790	4	336001	5	NULL	NULL	0	NULL	ceramide	Chemical	apoptotic capacity of	abolished by		selectively			sn-1,2-substituted diglyceride	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_259	8626522	Thus, the findings that  the apoptotic capacity of ceramide was ( a) comparably  augmented by both D- and L- forms of  erythro-sphingosine and  threo-sphingosine, but ( b) selectively abolished by  sn-1,2-substituted (but  not  sn-2,3-substituted or  rac-1,3-substituted) forms  of diglyceride additionally supports an involvement of PKC activity in  the reciprocal modulation of ceramide action by sphingosine and  diglyceride.	transcription
59791	5	336001	5	NULL	NULL	0	NULL	ceramide	Chemical	apoptotic capacity of	not abolished by					sn-2,3-substituted diglyceride	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_259	8626522	Thus, the findings that  the apoptotic capacity of ceramide was ( a) comparably  augmented by both D- and L- forms of  erythro-sphingosine and  threo-sphingosine, but ( b) selectively abolished by  sn-1,2-substituted (but  not  sn-2,3-substituted or  rac-1,3-substituted) forms  of diglyceride additionally supports an involvement of PKC activity in  the reciprocal modulation of ceramide action by sphingosine and  diglyceride.	transcription
59792	6	336001	5	NULL	NULL	0	NULL	ceramide	Chemical	apoptotic capacity of	not abolished by					rac-1,3-substituted diglyceride	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_259	8626522	Thus, the findings that  the apoptotic capacity of ceramide was ( a) comparably  augmented by both D- and L- forms of  erythro-sphingosine and  threo-sphingosine, but ( b) selectively abolished by  sn-1,2-substituted (but  not  sn-2,3-substituted or  rac-1,3-substituted) forms  of diglyceride additionally supports an involvement of PKC activity in  the reciprocal modulation of ceramide action by sphingosine and  diglyceride.	transcription
59793	7	336001	5	NULL	NULL	0	NULL	statement 5	Process		is an alternative to					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_259	8626522	Thus, the findings that  the apoptotic capacity of ceramide was ( a) comparably  augmented by both D- and L- forms of  erythro-sphingosine and  threo-sphingosine, but ( b) selectively abolished by  sn-1,2-substituted (but  not  sn-2,3-substituted or  rac-1,3-substituted) forms  of diglyceride additionally supports an involvement of PKC activity in  the reciprocal modulation of ceramide action by sphingosine and  diglyceride.	transcription
59794	8	336001	5	NULL	NULL	0	NULL	sphingosine	Chemical		modulate		reciprocally			ceramide	Chemical	action of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_259	8626522	Thus, the findings that  the apoptotic capacity of ceramide was ( a) comparably  augmented by both D- and L- forms of  erythro-sphingosine and  threo-sphingosine, but ( b) selectively abolished by  sn-1,2-substituted (but  not  sn-2,3-substituted or  rac-1,3-substituted) forms  of diglyceride additionally supports an involvement of PKC activity in  the reciprocal modulation of ceramide action by sphingosine and  diglyceride.	transcription
59795	9	336001	5	NULL	NULL	0	NULL	diglyceride	Chemical		modulate		reciprocally			ceramide	Chemical	action of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_259	8626522	Thus, the findings that  the apoptotic capacity of ceramide was ( a) comparably  augmented by both D- and L- forms of  erythro-sphingosine and  threo-sphingosine, but ( b) selectively abolished by  sn-1,2-substituted (but  not  sn-2,3-substituted or  rac-1,3-substituted) forms  of diglyceride additionally supports an involvement of PKC activity in  the reciprocal modulation of ceramide action by sphingosine and  diglyceride.	transcription
59796	10	336001	5	NULL	NULL	0	NULL	PKC	GP	activity of	is involved in					statement 8	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_259	8626522	Thus, the findings that  the apoptotic capacity of ceramide was ( a) comparably  augmented by both D- and L- forms of  erythro-sphingosine and  threo-sphingosine, but ( b) selectively abolished by  sn-1,2-substituted (but  not  sn-2,3-substituted or  rac-1,3-substituted) forms  of diglyceride additionally supports an involvement of PKC activity in  the reciprocal modulation of ceramide action by sphingosine and  diglyceride.	transcription
59797	11	336001	5	NULL	NULL	0	NULL	PKC	GP	activity of	is involved in					statement 9	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_259	8626522	Thus, the findings that  the apoptotic capacity of ceramide was ( a) comparably  augmented by both D- and L- forms of  erythro-sphingosine and  threo-sphingosine, but ( b) selectively abolished by  sn-1,2-substituted (but  not  sn-2,3-substituted or  rac-1,3-substituted) forms  of diglyceride additionally supports an involvement of PKC activity in  the reciprocal modulation of ceramide action by sphingosine and  diglyceride.	transcription
78887	1	336001	6	NULL	NULL	0	NULL	ceramide	Chemical		plays a role in					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_259	8626522	Thus, the findings that  the apoptotic capacity of ceramide was ( a) comparably  augmented by both D- and L- forms of  erythro-sphingosine and  threo-sphingosine, but ( b) selectively abolished by  sn-1,2-substituted (but  not  sn-2,3-substituted or  rac-1,3-substituted) forms  of diglyceride additionally supports an involvement of PKC activity in  the reciprocal modulation of ceramide action by sphingosine and  diglyceride.	transcription
78888	2	336001	6	NULL	NULL	0	NULL	statement 1	Process		is augmented by					erythro-sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_259	8626522	Thus, the findings that  the apoptotic capacity of ceramide was ( a) comparably  augmented by both D- and L- forms of  erythro-sphingosine and  threo-sphingosine, but ( b) selectively abolished by  sn-1,2-substituted (but  not  sn-2,3-substituted or  rac-1,3-substituted) forms  of diglyceride additionally supports an involvement of PKC activity in  the reciprocal modulation of ceramide action by sphingosine and  diglyceride.	transcription
78889	3	336001	6	NULL	NULL	0	NULL	statement 1	Process		is augmented by					threo-sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_259	8626522	Thus, the findings that  the apoptotic capacity of ceramide was ( a) comparably  augmented by both D- and L- forms of  erythro-sphingosine and  threo-sphingosine, but ( b) selectively abolished by  sn-1,2-substituted (but  not  sn-2,3-substituted or  rac-1,3-substituted) forms  of diglyceride additionally supports an involvement of PKC activity in  the reciprocal modulation of ceramide action by sphingosine and  diglyceride.	transcription
59798	1	336002	5	NULL	NULL	0	NULL	PAK1	GP		is activated by					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8137_s_6	9525917	We observed concentration- and time-dependent activation of PAK1 by sphingosine and several related long chain sphingoid bases but not by ceramides or a variety of other lipids.	transcription
59799	2	336002	5	NULL	NULL	0	NULL	statement 1	Process		is dependent on					concentration	QuantityOrMeasure				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8137_s_6	9525917	We observed concentration- and time-dependent activation of PAK1 by sphingosine and several related long chain sphingoid bases but not by ceramides or a variety of other lipids.	transcription
59800	3	336002	5	NULL	NULL	0	NULL	statement 1	Process		is dependent on					time	Time				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8137_s_6	9525917	We observed concentration- and time-dependent activation of PAK1 by sphingosine and several related long chain sphingoid bases but not by ceramides or a variety of other lipids.	transcription
59801	4	336002	5	NULL	NULL	0	NULL	PAK1	GP		is activated by					sphingoid bases	Chemical	sphingosine related;;long chain			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8137_s_6	9525917	We observed concentration- and time-dependent activation of PAK1 by sphingosine and several related long chain sphingoid bases but not by ceramides or a variety of other lipids.	transcription
59802	5	336002	5	NULL	NULL	0	NULL	statement 4	Process		is dependent on					concentration	QuantityOrMeasure				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8137_s_6	9525917	We observed concentration- and time-dependent activation of PAK1 by sphingosine and several related long chain sphingoid bases but not by ceramides or a variety of other lipids.	transcription
59803	6	336002	5	NULL	NULL	0	NULL	statement 4	Process		is dependent on					time	Time				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8137_s_6	9525917	We observed concentration- and time-dependent activation of PAK1 by sphingosine and several related long chain sphingoid bases but not by ceramides or a variety of other lipids.	transcription
59804	7	336002	5	NULL	NULL	0	NULL	PAK1	GP		is not activated by					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8137_s_6	9525917	We observed concentration- and time-dependent activation of PAK1 by sphingosine and several related long chain sphingoid bases but not by ceramides or a variety of other lipids.	transcription
59805	8	336002	5	NULL	NULL	0	NULL	PAK1	GP		is not activated by					lipids	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8137_s_6	9525917	We observed concentration- and time-dependent activation of PAK1 by sphingosine and several related long chain sphingoid bases but not by ceramides or a variety of other lipids.	transcription
78886	1	336002	6	NULL	NULL	0	NULL	sphingosine	Chemical		activates					PAK1	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8137_s_6	9525917	We observed concentration- and time-dependent activation of PAK1 by sphingosine and several related long chain sphingoid bases but not by ceramides or a variety of other lipids.	transcription
59806	1	336004	5	NULL	NULL	0	NULL	sphingosine	Chemical		acylated to					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34290_s_5	15180992	To determine whether the inhibitory effect on EGF-induced migration was because of decreased S1P or increased ceramide as a consequence of acylation of increased sphingosine by ceramide synthase, we used fumonisin B1, a specific inhibitor of ceramide synthase.	transcription
59807	2	336004	5	NULL	NULL	0	NULL	ceramide synthase	GP		catalyzes					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34290_s_5	15180992	To determine whether the inhibitory effect on EGF-induced migration was because of decreased S1P or increased ceramide as a consequence of acylation of increased sphingosine by ceramide synthase, we used fumonisin B1, a specific inhibitor of ceramide synthase.	transcription
59808	3	336004	5	NULL	NULL	0	NULL	fumonisin B1			is an inhibitor of		specific			ceramide synthase					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34290_s_5	15180992	To determine whether the inhibitory effect on EGF-induced migration was because of decreased S1P or increased ceramide as a consequence of acylation of increased sphingosine by ceramide synthase, we used fumonisin B1, a specific inhibitor of ceramide synthase.	transcription
78884	1	336004	6	NULL	NULL	0	NULL	fumonisin B1	Chemical		inhibits					ceramide synthase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34290_s_5	15180992	To determine whether the inhibitory effect on EGF-induced migration was because of decreased S1P or increased ceramide as a consequence of acylation of increased sphingosine by ceramide synthase, we used fumonisin B1, a specific inhibitor of ceramide synthase.	transcription
78885	2	336004	6	NULL	NULL	0	NULL	ceramide synthase	GP		increases					sphingosine	Chemical	acylation of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34290_s_5	15180992	To determine whether the inhibitory effect on EGF-induced migration was because of decreased S1P or increased ceramide as a consequence of acylation of increased sphingosine by ceramide synthase, we used fumonisin B1, a specific inhibitor of ceramide synthase.	transcription
59835	1	336005	5	NULL	NULL	0	NULL	ceramide	Chemical		bind		directly;;specific			CTSD	GP				NULL		0	NULL	NULL	NULL	gw60_embo_18_19_5252_s_68	10508159	Direct and specific binding of ceramide to CTSD was additionally assessed using the radiolabeled photo-crosslinking ceramide analog, 3-trifluoromethyl-3-( m-iodophenyl) diazirine D- erythro-sphingosine ([125]TID-ceramide) as the ligand (Weber and Brunner, 1995  ).	transcription
78883	1	336005	6	NULL	NULL	0	NULL	ceramide	Chemical		bind					CTSD	GP				NULL		0	NULL	NULL	NULL	gw60_embo_18_19_5252_s_68	10508159	Direct and specific binding of ceramide to CTSD was additionally assessed using the radiolabeled photo-crosslinking ceramide analog, 3-trifluoromethyl-3-( m-iodophenyl) diazirine D- erythro-sphingosine ([125]TID-ceramide) as the ligand (Weber and Brunner, 1995  ).	transcription
59836	1	336006	5	NULL	NULL	0	NULL	ceramide	Chemical		bind					CTSD	GP				NULL		0	NULL	NULL	NULL	gw60_embo_18_19_5252_s_71	10508159	Labeling of CTSD with [125]TID-ceramide allowed us to perform specificity analysis of ceramide binding to CTSD using different ceramide and sphingosine isomers and various unrelated lipids.	transcription
59837	1	336007	5	NULL	NULL	0	NULL	ceramide	Chemical		does not originate from					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12724_s_10	11821388	A rise in total ceramide levels was also observed; however, ceramide did not originate from [3]sphingosine, and S1P-induced apoptosis was not inhibited by fumonisin B, precluding involvement of  de novo ceramide synthesis in apoptosis.	transcription
59838	2	336007	5	NULL	NULL	0	NULL	apoptosis	Process		is induced by					S1P	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12724_s_10	11821388	A rise in total ceramide levels was also observed; however, ceramide did not originate from [3]sphingosine, and S1P-induced apoptosis was not inhibited by fumonisin B, precluding involvement of  de novo ceramide synthesis in apoptosis.	transcription
59839	3	336007	5	NULL	NULL	0	NULL	fumonisin B	Chemical		does not inhibit					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12724_s_10	11821388	A rise in total ceramide levels was also observed; however, ceramide did not originate from [3]sphingosine, and S1P-induced apoptosis was not inhibited by fumonisin B, precluding involvement of  de novo ceramide synthesis in apoptosis.	transcription
59840	4	336007	5	NULL	NULL	0	NULL	ceramide	Chemical	de novo synthesis of	is not involved in					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12724_s_10	11821388	A rise in total ceramide levels was also observed; however, ceramide did not originate from [3]sphingosine, and S1P-induced apoptosis was not inhibited by fumonisin B, precluding involvement of  de novo ceramide synthesis in apoptosis.	transcription
78881	1	336007	6	NULL	NULL	0	NULL	ceramide	Chemical		does not originate from					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12724_s_10	11821388	A rise in total ceramide levels was also observed; however, ceramide did not originate from [3]sphingosine, and S1P-induced apoptosis was not inhibited by fumonisin B, precluding involvement of  de novo ceramide synthesis in apoptosis.	transcription
78882	2	336007	6	NULL	NULL	0	NULL	fumonisin B	Chemical		does not inhibit					S1P-induced apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12724_s_10	11821388	A rise in total ceramide levels was also observed; however, ceramide did not originate from [3]sphingosine, and S1P-induced apoptosis was not inhibited by fumonisin B, precluding involvement of  de novo ceramide synthesis in apoptosis.	transcription
59841	1	336008	5	NULL	NULL	0	NULL	ceramide	Chemical	levels of	is regulated in		tightly			DCs	Cell	human			NULL		0	NULL	NULL	NULL	abs-batch0560-0569_j-leukoc-biol_79_1_16244104_s_4	16244104	We found  that ceramide levels are tightly regulated in human DCs and that the pharmacological  inhibition of enzymes responsible for ceramide catabolism, such as ceramidases  and sphingosine kinases, sensitizes DCs to ceramide-induced cell death.	transcription
59842	2	336008	5	NULL	NULL	0	NULL	cell death	Process		is induced by					ceramide	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0560-0569_j-leukoc-biol_79_1_16244104_s_4	16244104	We found  that ceramide levels are tightly regulated in human DCs and that the pharmacological  inhibition of enzymes responsible for ceramide catabolism, such as ceramidases  and sphingosine kinases, sensitizes DCs to ceramide-induced cell death.	transcription
59843	3	336008	5	NULL	NULL	0	NULL	ceramidases	GP		is responsible for					ceramide	Chemical	catabolism of			NULL		0	NULL	NULL	NULL	abs-batch0560-0569_j-leukoc-biol_79_1_16244104_s_4	16244104	We found  that ceramide levels are tightly regulated in human DCs and that the pharmacological  inhibition of enzymes responsible for ceramide catabolism, such as ceramidases  and sphingosine kinases, sensitizes DCs to ceramide-induced cell death.	transcription
59844	4	336008	5	NULL	NULL	0	NULL	sphingosine kinases	GP		is responsible for					ceramide	Chemical	catabolism of			NULL		0	NULL	NULL	NULL	abs-batch0560-0569_j-leukoc-biol_79_1_16244104_s_4	16244104	We found  that ceramide levels are tightly regulated in human DCs and that the pharmacological  inhibition of enzymes responsible for ceramide catabolism, such as ceramidases  and sphingosine kinases, sensitizes DCs to ceramide-induced cell death.	transcription
59845	5	336008	5	NULL	NULL	0	NULL	DCs	Cell	human	is sensitive to					statement 2	Process				NULL		0	NULL	NULL	NULL	abs-batch0560-0569_j-leukoc-biol_79_1_16244104_s_4	16244104	We found  that ceramide levels are tightly regulated in human DCs and that the pharmacological  inhibition of enzymes responsible for ceramide catabolism, such as ceramidases  and sphingosine kinases, sensitizes DCs to ceramide-induced cell death.	transcription
59846	6	336008	5	NULL	NULL	0	NULL	ceramidases	GP	pharmacological inhibition of	results in					statement 5	Process				NULL		0	NULL	NULL	NULL	abs-batch0560-0569_j-leukoc-biol_79_1_16244104_s_4	16244104	We found  that ceramide levels are tightly regulated in human DCs and that the pharmacological  inhibition of enzymes responsible for ceramide catabolism, such as ceramidases  and sphingosine kinases, sensitizes DCs to ceramide-induced cell death.	transcription
59847	7	336008	5	NULL	NULL	0	NULL	sphingosine kinase	GP	pharmacological inhibition of	results in					statement 5	Process				NULL		0	NULL	NULL	NULL	abs-batch0560-0569_j-leukoc-biol_79_1_16244104_s_4	16244104	We found  that ceramide levels are tightly regulated in human DCs and that the pharmacological  inhibition of enzymes responsible for ceramide catabolism, such as ceramidases  and sphingosine kinases, sensitizes DCs to ceramide-induced cell death.	transcription
78880	1	336008	6	NULL	NULL	0	NULL	ceramide	Chemical	levels of	are regulated in					DC	cell	human			NULL		0	NULL	NULL	NULL	abs-batch0560-0569_j-leukoc-biol_79_1_16244104_s_4	16244104	We found  that ceramide levels are tightly regulated in human DCs and that the pharmacological  inhibition of enzymes responsible for ceramide catabolism, such as ceramidases  and sphingosine kinases, sensitizes DCs to ceramide-induced cell death.	transcription
59848	1	336009	5	NULL	NULL	0	NULL	C -ceramide	Chemical		stimulates					Sphingosine 1-Phosphate	Chemical	metabolism of			NULL	fibroblasts	NULL	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_208	7592842	C  -ceramide Stimulates the Metabolism of  Sphingosine 1-Phosphate by FibroblastsRecently, we  demonstrated that at least part of the mechanism by which ceramides  block the effects of PA and lyso-PA on the stimulation of DNA synthesis  and PLD activity is by interfering with the interaction of the latter  two mitogens with the cells and by increasing their rates of metabolism ( 20) .	transcription
59869	2	336009	5	NULL	NULL	0	NULL	PA	Chemical		stimulates					DNA	NucleicAcid	synthesis of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_208	7592842	C  -ceramide Stimulates the Metabolism of  Sphingosine 1-Phosphate by FibroblastsRecently, we  demonstrated that at least part of the mechanism by which ceramides  block the effects of PA and lyso-PA on the stimulation of DNA synthesis  and PLD activity is by interfering with the interaction of the latter  two mitogens with the cells and by increasing their rates of metabolism ( 20) .	transcription
59870	3	336009	5	NULL	NULL	0	NULL	lyso-PA	Chemical		stimulates					DNA	NucleicAcid	synthesis of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_208	7592842	C  -ceramide Stimulates the Metabolism of  Sphingosine 1-Phosphate by FibroblastsRecently, we  demonstrated that at least part of the mechanism by which ceramides  block the effects of PA and lyso-PA on the stimulation of DNA synthesis  and PLD activity is by interfering with the interaction of the latter  two mitogens with the cells and by increasing their rates of metabolism ( 20) .	transcription
59871	4	336009	5	NULL	NULL	0	NULL	ceramide	Chemical		blocks					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_208	7592842	C  -ceramide Stimulates the Metabolism of  Sphingosine 1-Phosphate by FibroblastsRecently, we  demonstrated that at least part of the mechanism by which ceramides  block the effects of PA and lyso-PA on the stimulation of DNA synthesis  and PLD activity is by interfering with the interaction of the latter  two mitogens with the cells and by increasing their rates of metabolism ( 20) .	transcription
59872	5	336009	5	NULL	NULL	0	NULL	ceramide	Chemical		blocks					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_208	7592842	C  -ceramide Stimulates the Metabolism of  Sphingosine 1-Phosphate by FibroblastsRecently, we  demonstrated that at least part of the mechanism by which ceramides  block the effects of PA and lyso-PA on the stimulation of DNA synthesis  and PLD activity is by interfering with the interaction of the latter  two mitogens with the cells and by increasing their rates of metabolism ( 20) .	transcription
59873	6	336009	5	NULL	NULL	0	NULL	PA	Chemical		stimulates					PLD	GP	activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_208	7592842	C  -ceramide Stimulates the Metabolism of  Sphingosine 1-Phosphate by FibroblastsRecently, we  demonstrated that at least part of the mechanism by which ceramides  block the effects of PA and lyso-PA on the stimulation of DNA synthesis  and PLD activity is by interfering with the interaction of the latter  two mitogens with the cells and by increasing their rates of metabolism ( 20) .	transcription
59874	7	336009	5	NULL	NULL	0	NULL	lyso-PA	Chemical		stimulates					PLD	GP	activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_208	7592842	C  -ceramide Stimulates the Metabolism of  Sphingosine 1-Phosphate by FibroblastsRecently, we  demonstrated that at least part of the mechanism by which ceramides  block the effects of PA and lyso-PA on the stimulation of DNA synthesis  and PLD activity is by interfering with the interaction of the latter  two mitogens with the cells and by increasing their rates of metabolism ( 20) .	transcription
59875	8	336009	5	NULL	NULL	0	NULL	ceramide	Chemical		blocks					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_208	7592842	C  -ceramide Stimulates the Metabolism of  Sphingosine 1-Phosphate by FibroblastsRecently, we  demonstrated that at least part of the mechanism by which ceramides  block the effects of PA and lyso-PA on the stimulation of DNA synthesis  and PLD activity is by interfering with the interaction of the latter  two mitogens with the cells and by increasing their rates of metabolism ( 20) .	transcription
59876	9	336009	5	NULL	NULL	0	NULL	ceramide	Chemical		blocks					statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_208	7592842	C  -ceramide Stimulates the Metabolism of  Sphingosine 1-Phosphate by FibroblastsRecently, we  demonstrated that at least part of the mechanism by which ceramides  block the effects of PA and lyso-PA on the stimulation of DNA synthesis  and PLD activity is by interfering with the interaction of the latter  two mitogens with the cells and by increasing their rates of metabolism ( 20) .	transcription
59877	10	336009	5	NULL	NULL	0	NULL	PA	Chemical		is a type of					mitogen	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_208	7592842	C  -ceramide Stimulates the Metabolism of  Sphingosine 1-Phosphate by FibroblastsRecently, we  demonstrated that at least part of the mechanism by which ceramides  block the effects of PA and lyso-PA on the stimulation of DNA synthesis  and PLD activity is by interfering with the interaction of the latter  two mitogens with the cells and by increasing their rates of metabolism ( 20) .	transcription
59878	11	336009	5	NULL	NULL	0	NULL	lyso-PA	Chemical		is a type of					mitogen	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_208	7592842	C  -ceramide Stimulates the Metabolism of  Sphingosine 1-Phosphate by FibroblastsRecently, we  demonstrated that at least part of the mechanism by which ceramides  block the effects of PA and lyso-PA on the stimulation of DNA synthesis  and PLD activity is by interfering with the interaction of the latter  two mitogens with the cells and by increasing their rates of metabolism ( 20) .	transcription
78875	1	336009	6	NULL	NULL	0	NULL	ceramide	Chemical		stimulates					Sphingosine 1-Phosphate	Chemical	metabolism of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_208	7592842	C  -ceramide Stimulates the Metabolism of  Sphingosine 1-Phosphate by FibroblastsRecently, we  demonstrated that at least part of the mechanism by which ceramides  block the effects of PA and lyso-PA on the stimulation of DNA synthesis  and PLD activity is by interfering with the interaction of the latter  two mitogens with the cells and by increasing their rates of metabolism ( 20) .	transcription
78876	2	336009	6	NULL	NULL	0	NULL	PA	Chemical		effects					DNA	NucleicAcid	synthesis of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_208	7592842	C  -ceramide Stimulates the Metabolism of  Sphingosine 1-Phosphate by FibroblastsRecently, we  demonstrated that at least part of the mechanism by which ceramides  block the effects of PA and lyso-PA on the stimulation of DNA synthesis  and PLD activity is by interfering with the interaction of the latter  two mitogens with the cells and by increasing their rates of metabolism ( 20) .	transcription
78877	3	336009	6	NULL	NULL	0	NULL	lyso-PA	Chemical		effects					PLD	GP	activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_208	7592842	C  -ceramide Stimulates the Metabolism of  Sphingosine 1-Phosphate by FibroblastsRecently, we  demonstrated that at least part of the mechanism by which ceramides  block the effects of PA and lyso-PA on the stimulation of DNA synthesis  and PLD activity is by interfering with the interaction of the latter  two mitogens with the cells and by increasing their rates of metabolism ( 20) .	transcription
78878	4	336009	6	NULL	NULL	0	NULL	ceramide	Chemical		blocks					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_208	7592842	C  -ceramide Stimulates the Metabolism of  Sphingosine 1-Phosphate by FibroblastsRecently, we  demonstrated that at least part of the mechanism by which ceramides  block the effects of PA and lyso-PA on the stimulation of DNA synthesis  and PLD activity is by interfering with the interaction of the latter  two mitogens with the cells and by increasing their rates of metabolism ( 20) .	transcription
78879	5	336009	6	NULL	NULL	0	NULL	ceramide	Chemical		blocks					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_208	7592842	C  -ceramide Stimulates the Metabolism of  Sphingosine 1-Phosphate by FibroblastsRecently, we  demonstrated that at least part of the mechanism by which ceramides  block the effects of PA and lyso-PA on the stimulation of DNA synthesis  and PLD activity is by interfering with the interaction of the latter  two mitogens with the cells and by increasing their rates of metabolism ( 20) .	transcription
59879	1	336010	5	NULL	NULL	0	NULL	sphingosine	Chemical		is converted to					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_83	10747891	It should be noted that similar to addition of sphingosine, treatment with C2-ceramide also resulted in the appearance of a late peak of endogenous ceramide (Fig.  2 B), which could be due in part to conversion of sphingosine (Fig.  1 B) to ceramide by ceramide synthase, inasmuch as fumonisin B1 was capable of inhibiting the late increase.	transcription
59880	2	336010	5	NULL	NULL	0	NULL	ceramide synthase	GP		catalyzes					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_83	10747891	It should be noted that similar to addition of sphingosine, treatment with C2-ceramide also resulted in the appearance of a late peak of endogenous ceramide (Fig.  2 B), which could be due in part to conversion of sphingosine (Fig.  1 B) to ceramide by ceramide synthase, inasmuch as fumonisin B1 was capable of inhibiting the late increase.	transcription
59881	3	336010	5	NULL	NULL	0	NULL	C2-ceramide	Chemical	treatment	results in					ceramide	Chemical	appearance of;;endogenous			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_83	10747891	It should be noted that similar to addition of sphingosine, treatment with C2-ceramide also resulted in the appearance of a late peak of endogenous ceramide (Fig.  2 B), which could be due in part to conversion of sphingosine (Fig.  1 B) to ceramide by ceramide synthase, inasmuch as fumonisin B1 was capable of inhibiting the late increase.	transcription
59882	4	336010	5	NULL	NULL	0	NULL	fumonisin B1	Chemical		inhibit					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_83	10747891	It should be noted that similar to addition of sphingosine, treatment with C2-ceramide also resulted in the appearance of a late peak of endogenous ceramide (Fig.  2 B), which could be due in part to conversion of sphingosine (Fig.  1 B) to ceramide by ceramide synthase, inasmuch as fumonisin B1 was capable of inhibiting the late increase.	transcription
78872	1	336010	6	NULL	NULL	0	NULL	sphingosine	Chemical		is converted to					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_83	10747891	It should be noted that similar to addition of sphingosine, treatment with C2-ceramide also resulted in the appearance of a late peak of endogenous ceramide (Fig.  2 B), which could be due in part to conversion of sphingosine (Fig.  1 B) to ceramide by ceramide synthase, inasmuch as fumonisin B1 was capable of inhibiting the late increase.	transcription
78873	2	336010	6	NULL	NULL	0	NULL	statement 1	Process		is catalyzed by					ceramide synthase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_83	10747891	It should be noted that similar to addition of sphingosine, treatment with C2-ceramide also resulted in the appearance of a late peak of endogenous ceramide (Fig.  2 B), which could be due in part to conversion of sphingosine (Fig.  1 B) to ceramide by ceramide synthase, inasmuch as fumonisin B1 was capable of inhibiting the late increase.	transcription
78874	3	336010	6	NULL	NULL	0	NULL	fumonisin B1	Chemical		inhibits					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_83	10747891	It should be noted that similar to addition of sphingosine, treatment with C2-ceramide also resulted in the appearance of a late peak of endogenous ceramide (Fig.  2 B), which could be due in part to conversion of sphingosine (Fig.  1 B) to ceramide by ceramide synthase, inasmuch as fumonisin B1 was capable of inhibiting the late increase.	transcription
59883	1	336011	5	NULL	NULL	0	NULL	sphingosine	Chemical		induce					growth suppression	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_21_12646_s_281	8647877	In many cell systems, sphingosine and  ceramide induce similar activities such as growth suppression, and  induction of Rb dephosphorylation( 37,  62) , whereas in  other situations, sphingosine may have effects opposite to those of  ceramide such as activation of phospholipase D ( 63,  64) which is inhibited by  ceramide( 65,  66,  67,  68,  69) .	transcription
59884	2	336011	5	NULL	NULL	0	NULL	ceramide	Chemical		induce					growth suppression	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_21_12646_s_281	8647877	In many cell systems, sphingosine and  ceramide induce similar activities such as growth suppression, and  induction of Rb dephosphorylation( 37,  62) , whereas in  other situations, sphingosine may have effects opposite to those of  ceramide such as activation of phospholipase D ( 63,  64) which is inhibited by  ceramide( 65,  66,  67,  68,  69) .	transcription
59885	3	336011	5	NULL	NULL	0	NULL	sphingosine	Chemical		induce					Rb	GP	dephosphorylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_21_12646_s_281	8647877	In many cell systems, sphingosine and  ceramide induce similar activities such as growth suppression, and  induction of Rb dephosphorylation( 37,  62) , whereas in  other situations, sphingosine may have effects opposite to those of  ceramide such as activation of phospholipase D ( 63,  64) which is inhibited by  ceramide( 65,  66,  67,  68,  69) .	transcription
59886	4	336011	5	NULL	NULL	0	NULL	ceramide	Chemical		induce					Rb	GP	dephosphorylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_21_12646_s_281	8647877	In many cell systems, sphingosine and  ceramide induce similar activities such as growth suppression, and  induction of Rb dephosphorylation( 37,  62) , whereas in  other situations, sphingosine may have effects opposite to those of  ceramide such as activation of phospholipase D ( 63,  64) which is inhibited by  ceramide( 65,  66,  67,  68,  69) .	transcription
59887	5	336011	5	NULL	NULL	0	NULL	sphingosine	Chemical		activates					phospholipase D	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_21_12646_s_281	8647877	In many cell systems, sphingosine and  ceramide induce similar activities such as growth suppression, and  induction of Rb dephosphorylation( 37,  62) , whereas in  other situations, sphingosine may have effects opposite to those of  ceramide such as activation of phospholipase D ( 63,  64) which is inhibited by  ceramide( 65,  66,  67,  68,  69) .	transcription
59888	6	336011	5	NULL	NULL	0	NULL	ceramide	Chemical		inhibit					phospholipase D	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_21_12646_s_281	8647877	In many cell systems, sphingosine and  ceramide induce similar activities such as growth suppression, and  induction of Rb dephosphorylation( 37,  62) , whereas in  other situations, sphingosine may have effects opposite to those of  ceramide such as activation of phospholipase D ( 63,  64) which is inhibited by  ceramide( 65,  66,  67,  68,  69) .	transcription
59889	1	336012	5	NULL	NULL	0	NULL	ceramide	Chemical		metabolized to		easily			sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_146	16936207	Because ceramide is easily metabolized to sphingosine, which, in turn, is readily converted to S1P, we also determined whether sphingosine and S1P can regulate the expression of proinflammatory cytokines in adipocytes ( Figs. 5 B -  E).	transcription
59890	2	336012	5	NULL	NULL	0	NULL	sphingosine	Chemical		is converted to		readily			S1P	Chemical				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_146	16936207	Because ceramide is easily metabolized to sphingosine, which, in turn, is readily converted to S1P, we also determined whether sphingosine and S1P can regulate the expression of proinflammatory cytokines in adipocytes ( Figs. 5 B -  E).	transcription
59891	3	336012	5	NULL	NULL	0	NULL	sphingosine	Chemical		regulates		potentially			cytokines	GP	expression of;;proinflammatory			NULL	adipocytes	0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_146	16936207	Because ceramide is easily metabolized to sphingosine, which, in turn, is readily converted to S1P, we also determined whether sphingosine and S1P can regulate the expression of proinflammatory cytokines in adipocytes ( Figs. 5 B -  E).	transcription
59892	4	336012	5	NULL	NULL	0	NULL	S1P	Chemical		regulates		potentially			cytokines	GP	expression of;;proinflammatory			NULL	adipocytes	NULL	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_146	16936207	Because ceramide is easily metabolized to sphingosine, which, in turn, is readily converted to S1P, we also determined whether sphingosine and S1P can regulate the expression of proinflammatory cytokines in adipocytes ( Figs. 5 B -  E).	transcription
78870	1	336012	6	NULL	NULL	0	NULL	ceramide	Chemical		is metabolized into					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_146	16936207	Because ceramide is easily metabolized to sphingosine, which, in turn, is readily converted to S1P, we also determined whether sphingosine and S1P can regulate the expression of proinflammatory cytokines in adipocytes ( Figs. 5 B -  E).	transcription
78871	2	336012	6	NULL	NULL	0	NULL	sphingosine	Chemical		is converted to					S1P	GP				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_146	16936207	Because ceramide is easily metabolized to sphingosine, which, in turn, is readily converted to S1P, we also determined whether sphingosine and S1P can regulate the expression of proinflammatory cytokines in adipocytes ( Figs. 5 B -  E).	transcription
59893	1	336013	5	NULL	NULL	0	NULL	gene transcription	Process		is mediated by									SRE	NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_943_s_167	15132973	32,36  SRE-mediated gene transcription and mature SREBP levels are increased when ceramide synthesis is increased by sphingosine either added exogenously or increased endogenously through inhibition of sphingosine kinase ( Figure 4).	transcription
59899	2	336013	5	NULL	NULL	0	NULL	sphingosine	Chemical	addition of;;exogenous	increases					ceramide	Chemical	synthesis of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_943_s_167	15132973	32,36  SRE-mediated gene transcription and mature SREBP levels are increased when ceramide synthesis is increased by sphingosine either added exogenously or increased endogenously through inhibition of sphingosine kinase ( Figure 4).	transcription
59901	3	336013	5	NULL	NULL	0	NULL	sphingosine kinase	Chemical		increases		endogenously			ceramide	Chemical	synthesis of			NULL		NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_943_s_167	15132973	32,36  SRE-mediated gene transcription and mature SREBP levels are increased when ceramide synthesis is increased by sphingosine either added exogenously or increased endogenously through inhibition of sphingosine kinase ( Figure 4).	transcription
59904	4	336013	5	NULL	NULL	0	NULL	statement 2	Process		increases					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_943_s_167	15132973	32,36  SRE-mediated gene transcription and mature SREBP levels are increased when ceramide synthesis is increased by sphingosine either added exogenously or increased endogenously through inhibition of sphingosine kinase ( Figure 4).	transcription
60048	5	336013	5	NULL	NULL	0	NULL	statement 3	Process		occurs through					sphingosine kinase	GP	inhibition of			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_943_s_167	15132973	32,36  SRE-mediated gene transcription and mature SREBP levels are increased when ceramide synthesis is increased by sphingosine either added exogenously or increased endogenously through inhibition of sphingosine kinase ( Figure 4).	transcription
60049	6	336013	5	NULL	NULL	0	NULL	statement 3	Process		increases					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_943_s_167	15132973	32,36  SRE-mediated gene transcription and mature SREBP levels are increased when ceramide synthesis is increased by sphingosine either added exogenously or increased endogenously through inhibition of sphingosine kinase ( Figure 4).	transcription
60050	7	336013	5	NULL	NULL	0	NULL	statement 2	Process		increases					SREBP	GP	level of;;mature			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_943_s_167	15132973	32,36  SRE-mediated gene transcription and mature SREBP levels are increased when ceramide synthesis is increased by sphingosine either added exogenously or increased endogenously through inhibition of sphingosine kinase ( Figure 4).	transcription
60051	8	336013	5	NULL	NULL	0	NULL	statement 3	Process		increases					SREBP	GP	level of;;mature			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_943_s_167	15132973	32,36  SRE-mediated gene transcription and mature SREBP levels are increased when ceramide synthesis is increased by sphingosine either added exogenously or increased endogenously through inhibition of sphingosine kinase ( Figure 4).	transcription
78867	1	336013	6	NULL	NULL	0	NULL	sphingosine	Chemical		increases					ceramide	Chemical	synthesis of 			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_943_s_167	15132973	32,36  SRE-mediated gene transcription and mature SREBP levels are increased when ceramide synthesis is increased by sphingosine either added exogenously or increased endogenously through inhibition of sphingosine kinase ( Figure 4).	transcription
78868	2	336013	6	NULL	NULL	0	NULL	statement 1	Process		increases					SREBP	GP	levels of 			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_943_s_167	15132973	32,36  SRE-mediated gene transcription and mature SREBP levels are increased when ceramide synthesis is increased by sphingosine either added exogenously or increased endogenously through inhibition of sphingosine kinase ( Figure 4).	transcription
78869	3	336013	6	NULL	NULL	0	NULL	sphingosine kinase	GP	inhibition of 	increases					ceramide	Chemical	synthesis of 			NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_24_5_943_s_167	15132973	32,36  SRE-mediated gene transcription and mature SREBP levels are increased when ceramide synthesis is increased by sphingosine either added exogenously or increased endogenously through inhibition of sphingosine kinase ( Figure 4).	transcription
60052	1	336014	5	NULL	NULL	0	NULL	TNF-alpha	GP		induce					ceramide	Chemical	change in;;level of			NULL	HUVECs	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_99_s_31	16269668	ctivation of N-SMase and sphingosine-kinase (SK) and changes in ceramide, sphingosine, and Sph1P levels induced by TNF-alpha are time dependent and precede activation of Akt and eNOS in HUVECs.	transcription
60053	2	336014	5	NULL	NULL	0	NULL	TNF-alpha	GP		induce					sphingosine	Chemical	change in;;level of			NULL	HUVECs	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_99_s_31	16269668	ctivation of N-SMase and sphingosine-kinase (SK) and changes in ceramide, sphingosine, and Sph1P levels induced by TNF-alpha are time dependent and precede activation of Akt and eNOS in HUVECs.	transcription
60054	3	336014	5	NULL	NULL	0	NULL	TNF-alpha	GP		induce					Sph1P	Chemical	change in;;level of			NULL	HUVECs	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_99_s_31	16269668	ctivation of N-SMase and sphingosine-kinase (SK) and changes in ceramide, sphingosine, and Sph1P levels induced by TNF-alpha are time dependent and precede activation of Akt and eNOS in HUVECs.	transcription
60055	4	336014	5	NULL	NULL	0	NULL	statement 1	Process		precede					Akt	GP	activation of			NULL	HUVECs	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_99_s_31	16269668	ctivation of N-SMase and sphingosine-kinase (SK) and changes in ceramide, sphingosine, and Sph1P levels induced by TNF-alpha are time dependent and precede activation of Akt and eNOS in HUVECs.	transcription
60056	5	336014	5	NULL	NULL	0	NULL	statement 1	Process		precede					eNOS	GP	activation of			NULL	HUVECs	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_99_s_31	16269668	ctivation of N-SMase and sphingosine-kinase (SK) and changes in ceramide, sphingosine, and Sph1P levels induced by TNF-alpha are time dependent and precede activation of Akt and eNOS in HUVECs.	transcription
60057	6	336014	5	NULL	NULL	0	NULL	statement 2	Process		precede					Akt	GP	activation of			NULL	HUVECs	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_99_s_31	16269668	ctivation of N-SMase and sphingosine-kinase (SK) and changes in ceramide, sphingosine, and Sph1P levels induced by TNF-alpha are time dependent and precede activation of Akt and eNOS in HUVECs.	transcription
60058	7	336014	5	NULL	NULL	0	NULL	statement 2	Process		precede					eNOS	GP	activation of			NULL	HUVECs	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_99_s_31	16269668	ctivation of N-SMase and sphingosine-kinase (SK) and changes in ceramide, sphingosine, and Sph1P levels induced by TNF-alpha are time dependent and precede activation of Akt and eNOS in HUVECs.	transcription
60059	8	336014	5	NULL	NULL	0	NULL	statement 3	Process		precede					Akt	GP	activation of			NULL	HUVECs	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_99_s_31	16269668	ctivation of N-SMase and sphingosine-kinase (SK) and changes in ceramide, sphingosine, and Sph1P levels induced by TNF-alpha are time dependent and precede activation of Akt and eNOS in HUVECs.	transcription
60060	9	336014	5	NULL	NULL	0	NULL	statement 3	Process		precede					eNOS	GP	activation of			NULL	HUVECs	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_99_s_31	16269668	ctivation of N-SMase and sphingosine-kinase (SK) and changes in ceramide, sphingosine, and Sph1P levels induced by TNF-alpha are time dependent and precede activation of Akt and eNOS in HUVECs.	transcription
60061	10	336014	5	NULL	NULL	0	NULL	N-SMase	GP	activation of	precede					Akt	GP	activation of			NULL	HUVECs	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_99_s_31	16269668	ctivation of N-SMase and sphingosine-kinase (SK) and changes in ceramide, sphingosine, and Sph1P levels induced by TNF-alpha are time dependent and precede activation of Akt and eNOS in HUVECs.	transcription
60062	11	336014	5	NULL	NULL	0	NULL	N-SMase	GP	activation of	precede					eNOS	GP	activation of			NULL	HUVECs	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_99_s_31	16269668	ctivation of N-SMase and sphingosine-kinase (SK) and changes in ceramide, sphingosine, and Sph1P levels induced by TNF-alpha are time dependent and precede activation of Akt and eNOS in HUVECs.	transcription
60063	12	336014	5	NULL	NULL	0	NULL	sphingosine-kinase	GP	activation of	precede					Akt	GP	activation of			NULL	HUVECs	NULL	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_99_s_31	16269668	ctivation of N-SMase and sphingosine-kinase (SK) and changes in ceramide, sphingosine, and Sph1P levels induced by TNF-alpha are time dependent and precede activation of Akt and eNOS in HUVECs.	transcription
60064	13	336014	5	NULL	NULL	0	NULL	sphingosine-kinase	GP	activation of	precede					eNOS	GP	activation of			NULL	HUVECs	0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_99_s_31	16269668	ctivation of N-SMase and sphingosine-kinase (SK) and changes in ceramide, sphingosine, and Sph1P levels induced by TNF-alpha are time dependent and precede activation of Akt and eNOS in HUVECs.	transcription
60065	14	336014	5	NULL	NULL	0	NULL	SK	GP		is					sphingosine kinase	GP				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_99_s_31	16269668	ctivation of N-SMase and sphingosine-kinase (SK) and changes in ceramide, sphingosine, and Sph1P levels induced by TNF-alpha are time dependent and precede activation of Akt and eNOS in HUVECs.	transcription
78864	1	336014	6	NULL	NULL	0	NULL	TNF-alpha	GP		induces					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_99_s_31	16269668	ctivation of N-SMase and sphingosine-kinase (SK) and changes in ceramide, sphingosine, and Sph1P levels induced by TNF-alpha are time dependent and precede activation of Akt and eNOS in HUVECs.	transcription
78865	2	336014	6	NULL	NULL	0	NULL	TNF-alpha	GP		induces					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_99_s_31	16269668	ctivation of N-SMase and sphingosine-kinase (SK) and changes in ceramide, sphingosine, and Sph1P levels induced by TNF-alpha are time dependent and precede activation of Akt and eNOS in HUVECs.	transcription
78866	3	336014	6	NULL	NULL	0	NULL	TNF-alpha	GP		induces					Sph1P	GP				NULL		0	NULL	NULL	NULL	gw70_arterthrombvascbiol_26_1_99_s_31	16269668	ctivation of N-SMase and sphingosine-kinase (SK) and changes in ceramide, sphingosine, and Sph1P levels induced by TNF-alpha are time dependent and precede activation of Akt and eNOS in HUVECs.	transcription
60066	1	336015	5	NULL	NULL	0	NULL	S1P	Chemical		is generated by					sphingosine kinase	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_36_34541_s_203	12815058	Tipping  the balance toward S1P generation by sphingosine kinase activation precludes  induction of apoptosis ( ),  whereas overexpression of SPPase leads to the breakdown of S1P into  sphingosine and ceramide, thereby promoting induction of apoptosis  ( ).	transcription
60067	2	336015	5	NULL	NULL	0	NULL	statement 1	Process		precludes					apoptosis	Process	induction of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_36_34541_s_203	12815058	Tipping  the balance toward S1P generation by sphingosine kinase activation precludes  induction of apoptosis ( ),  whereas overexpression of SPPase leads to the breakdown of S1P into  sphingosine and ceramide, thereby promoting induction of apoptosis  ( ).	transcription
60068	3	336015	5	NULL	NULL	0	NULL	S1P	Chemical		broken down into					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_36_34541_s_203	12815058	Tipping  the balance toward S1P generation by sphingosine kinase activation precludes  induction of apoptosis ( ),  whereas overexpression of SPPase leads to the breakdown of S1P into  sphingosine and ceramide, thereby promoting induction of apoptosis  ( ).	transcription
60069	4	336015	5	NULL	NULL	0	NULL	S1P	Chemical		broken down into					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_36_34541_s_203	12815058	Tipping  the balance toward S1P generation by sphingosine kinase activation precludes  induction of apoptosis ( ),  whereas overexpression of SPPase leads to the breakdown of S1P into  sphingosine and ceramide, thereby promoting induction of apoptosis  ( ).	transcription
60070	5	336015	5	NULL	NULL	0	NULL	statement 3	Process		occurs along with					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_36_34541_s_203	12815058	Tipping  the balance toward S1P generation by sphingosine kinase activation precludes  induction of apoptosis ( ),  whereas overexpression of SPPase leads to the breakdown of S1P into  sphingosine and ceramide, thereby promoting induction of apoptosis  ( ).	transcription
60071	6	336015	5	NULL	NULL	0	NULL	SPPase	GP	overexpression of	leads to					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_36_34541_s_203	12815058	Tipping  the balance toward S1P generation by sphingosine kinase activation precludes  induction of apoptosis ( ),  whereas overexpression of SPPase leads to the breakdown of S1P into  sphingosine and ceramide, thereby promoting induction of apoptosis  ( ).	transcription
60072	7	336015	5	NULL	NULL	0	NULL	statement 6	Process		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_36_34541_s_203	12815058	Tipping  the balance toward S1P generation by sphingosine kinase activation precludes  induction of apoptosis ( ),  whereas overexpression of SPPase leads to the breakdown of S1P into  sphingosine and ceramide, thereby promoting induction of apoptosis  ( ).	transcription
78858	1	336015	6	NULL	NULL	NULL	NULL	sphingosine kinase	GP	activation of	generates					S1P	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_36_34541_s_203	12815058	Tipping  the balance toward S1P generation by sphingosine kinase activation precludes  induction of apoptosis ( ),  whereas overexpression of SPPase leads to the breakdown of S1P into  sphingosine and ceramide, thereby promoting induction of apoptosis  ( ).	transcription
78859	2	336015	6	NULL	NULL	0	NULL	statement 1	Process		precludes					apoptosis	Process	induction of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_36_34541_s_203	12815058	Tipping  the balance toward S1P generation by sphingosine kinase activation precludes  induction of apoptosis ( ),  whereas overexpression of SPPase leads to the breakdown of S1P into  sphingosine and ceramide, thereby promoting induction of apoptosis  ( ).	transcription
78860	3	336015	6	NULL	NULL	0	NULL	S1P	GP		generates					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_36_34541_s_203	12815058	Tipping  the balance toward S1P generation by sphingosine kinase activation precludes  induction of apoptosis ( ),  whereas overexpression of SPPase leads to the breakdown of S1P into  sphingosine and ceramide, thereby promoting induction of apoptosis  ( ).	transcription
78861	4	336015	6	NULL	NULL	0	NULL	S1P	Chemical		generates					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_36_34541_s_203	12815058	Tipping  the balance toward S1P generation by sphingosine kinase activation precludes  induction of apoptosis ( ),  whereas overexpression of SPPase leads to the breakdown of S1P into  sphingosine and ceramide, thereby promoting induction of apoptosis  ( ).	transcription
78862	6	336015	6	NULL	NULL	0	NULL	SPPase	GP	overexpression of	leads to					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_36_34541_s_203	12815058	Tipping  the balance toward S1P generation by sphingosine kinase activation precludes  induction of apoptosis ( ),  whereas overexpression of SPPase leads to the breakdown of S1P into  sphingosine and ceramide, thereby promoting induction of apoptosis  ( ).	transcription
78863	5	336015	6	NULL	NULL	0	NULL	statement 3	Process		occurs simultaneously with					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_36_34541_s_203	12815058	Tipping  the balance toward S1P generation by sphingosine kinase activation precludes  induction of apoptosis ( ),  whereas overexpression of SPPase leads to the breakdown of S1P into  sphingosine and ceramide, thereby promoting induction of apoptosis  ( ).	transcription
60073	1	336016	5	NULL	NULL	0	NULL	SPC	Chemical		is an analog of					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_317_2_685_s_113	16415087	Of the sphingosine analogs tested, SPC and dihydrosphingosine 1-phosphate (at concentrations of 5 muM) were as effective as S1P, whereas the addition of sphingosine, dihydrosphingosine, dimethylsphingosine, or ceramide had little or no effect on taurine efflux ( Table 1).	transcription
60074	2	336016	5	NULL	NULL	0	NULL	dihydrosphingosine 1-phosphate	Chemical		is an analog of					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_317_2_685_s_113	16415087	Of the sphingosine analogs tested, SPC and dihydrosphingosine 1-phosphate (at concentrations of 5 muM) were as effective as S1P, whereas the addition of sphingosine, dihydrosphingosine, dimethylsphingosine, or ceramide had little or no effect on taurine efflux ( Table 1).	transcription
60075	3	336016	5	NULL	NULL	0	NULL	SPC	Chemical		is as effective as					S1P	Chemical				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_317_2_685_s_113	16415087	Of the sphingosine analogs tested, SPC and dihydrosphingosine 1-phosphate (at concentrations of 5 muM) were as effective as S1P, whereas the addition of sphingosine, dihydrosphingosine, dimethylsphingosine, or ceramide had little or no effect on taurine efflux ( Table 1).	transcription
60076	4	336016	5	NULL	NULL	0	NULL	dihydrosphingosine 1-phosphate	Chemical		is as effective as					S1P	Chemical				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_317_2_685_s_113	16415087	Of the sphingosine analogs tested, SPC and dihydrosphingosine 1-phosphate (at concentrations of 5 muM) were as effective as S1P, whereas the addition of sphingosine, dihydrosphingosine, dimethylsphingosine, or ceramide had little or no effect on taurine efflux ( Table 1).	transcription
60077	5	336016	5	NULL	NULL	0	NULL	sphingosine	Chemical		does not effect					taurine	Chemical	efflux of			NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_317_2_685_s_113	16415087	Of the sphingosine analogs tested, SPC and dihydrosphingosine 1-phosphate (at concentrations of 5 muM) were as effective as S1P, whereas the addition of sphingosine, dihydrosphingosine, dimethylsphingosine, or ceramide had little or no effect on taurine efflux ( Table 1).	transcription
60091	6	336016	5	NULL	NULL	0	NULL	dihydrosphingosine	Chemical		does not effect					taurine	Chemical	efflux of			NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_317_2_685_s_113	16415087	Of the sphingosine analogs tested, SPC and dihydrosphingosine 1-phosphate (at concentrations of 5 muM) were as effective as S1P, whereas the addition of sphingosine, dihydrosphingosine, dimethylsphingosine, or ceramide had little or no effect on taurine efflux ( Table 1).	transcription
60092	7	336016	5	NULL	NULL	0	NULL	dimethylsphingosine	Chemical		does not effect					taurine	Chemical	efflux of			NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_317_2_685_s_113	16415087	Of the sphingosine analogs tested, SPC and dihydrosphingosine 1-phosphate (at concentrations of 5 muM) were as effective as S1P, whereas the addition of sphingosine, dihydrosphingosine, dimethylsphingosine, or ceramide had little or no effect on taurine efflux ( Table 1).	transcription
60093	8	336016	5	NULL	NULL	0	NULL	ceramide	Chemical		does not effect					taurine	Chemical	efflux of			NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_317_2_685_s_113	16415087	Of the sphingosine analogs tested, SPC and dihydrosphingosine 1-phosphate (at concentrations of 5 muM) were as effective as S1P, whereas the addition of sphingosine, dihydrosphingosine, dimethylsphingosine, or ceramide had little or no effect on taurine efflux ( Table 1).	transcription
60101	1	336018	5	NULL	NULL	0	NULL	ceramide	Chemical		is synthesized from					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_febslett_425_1_61_s_48	9541007	As we previously reported [ 8, blocking ceramide synthesis from sphingosine by the addition of the fungal agent Fumonisin B1 (25  M) did not inhibit sphingosine from inducing apoptosis ( Fig. 1A).	transcription
60102	2	336018	5	NULL	NULL	0	NULL	Fumonisin B1	Chemical		blocks					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_425_1_61_s_48	9541007	As we previously reported [ 8, blocking ceramide synthesis from sphingosine by the addition of the fungal agent Fumonisin B1 (25  M) did not inhibit sphingosine from inducing apoptosis ( Fig. 1A).	transcription
60103	3	336018	5	NULL	NULL	0	NULL	Fumonisin B1	Chemical		is a type of					fungal agent	Chemical				NULL		0	NULL	NULL	NULL	gw60_febslett_425_1_61_s_48	9541007	As we previously reported [ 8, blocking ceramide synthesis from sphingosine by the addition of the fungal agent Fumonisin B1 (25  M) did not inhibit sphingosine from inducing apoptosis ( Fig. 1A).	transcription
60104	4	336018	5	NULL	NULL	0	NULL	sphingosine	Chemical		induce					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_febslett_425_1_61_s_48	9541007	As we previously reported [ 8, blocking ceramide synthesis from sphingosine by the addition of the fungal agent Fumonisin B1 (25  M) did not inhibit sphingosine from inducing apoptosis ( Fig. 1A).	transcription
60105	5	336018	5	NULL	NULL	0	NULL	statement 2	Process		does not inhibit					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_425_1_61_s_48	9541007	As we previously reported [ 8, blocking ceramide synthesis from sphingosine by the addition of the fungal agent Fumonisin B1 (25  M) did not inhibit sphingosine from inducing apoptosis ( Fig. 1A).	transcription
78847	1	336018	6	NULL	NULL	0	NULL	sphingosine	Chemical		induces					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_425_1_61_s_48	9541007	As we previously reported [ 8, blocking ceramide synthesis from sphingosine by the addition of the fungal agent Fumonisin B1 (25  M) did not inhibit sphingosine from inducing apoptosis ( Fig. 1A).	transcription
78848	2	336018	6	NULL	NULL	0	NULL	sphingosine 	Chemical		induces					ceramide	Chemical	synthesis of 			NULL		0	NULL	NULL	NULL	gw60_febslett_425_1_61_s_48	9541007	As we previously reported [ 8, blocking ceramide synthesis from sphingosine by the addition of the fungal agent Fumonisin B1 (25  M) did not inhibit sphingosine from inducing apoptosis ( Fig. 1A).	transcription
78849	3	336018	6	NULL	NULL	0	NULL	Fumonisin B1	Chemical		blocks					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_425_1_61_s_48	9541007	As we previously reported [ 8, blocking ceramide synthesis from sphingosine by the addition of the fungal agent Fumonisin B1 (25  M) did not inhibit sphingosine from inducing apoptosis ( Fig. 1A).	transcription
78850	4	336018	6	NULL	NULL	0	NULL	statement 3	Process		does not inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_425_1_61_s_48	9541007	As we previously reported [ 8, blocking ceramide synthesis from sphingosine by the addition of the fungal agent Fumonisin B1 (25  M) did not inhibit sphingosine from inducing apoptosis ( Fig. 1A).	transcription
60106	1	336019	5	NULL	NULL	0	NULL	ceramide	Chemical		is converted to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_126_1_189_s_170	10051135	Therefore there appears to be a link between the sphingosine and cyclo-oxygenase pathways in the TNF-mediated coronary constriction, but the direct cardiac depressant actions of TNF are dependant on the conversion of ceramide of sphingosine, and do not involve the cyclo-oxygenase pathway.	transcription
60107	2	336019	5	NULL	NULL	0	NULL	TNF	GP	direct cardiac depressant actions of	is dependent on					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_126_1_189_s_170	10051135	Therefore there appears to be a link between the sphingosine and cyclo-oxygenase pathways in the TNF-mediated coronary constriction, but the direct cardiac depressant actions of TNF are dependant on the conversion of ceramide of sphingosine, and do not involve the cyclo-oxygenase pathway.	transcription
60108	3	336019	5	NULL	NULL	0	NULL	TNF	GP	direct cardiac depressant actions of	does not involve					cyclo-oxygenase pathway	Process				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_126_1_189_s_170	10051135	Therefore there appears to be a link between the sphingosine and cyclo-oxygenase pathways in the TNF-mediated coronary constriction, but the direct cardiac depressant actions of TNF are dependant on the conversion of ceramide of sphingosine, and do not involve the cyclo-oxygenase pathway.	transcription
60109	4	336019	5	NULL	NULL	0	NULL	TNF	GP		mediates					coronary constriction	Process				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_126_1_189_s_170	10051135	Therefore there appears to be a link between the sphingosine and cyclo-oxygenase pathways in the TNF-mediated coronary constriction, but the direct cardiac depressant actions of TNF are dependant on the conversion of ceramide of sphingosine, and do not involve the cyclo-oxygenase pathway.	transcription
60110	5	336019	5	NULL	NULL	0	NULL	sphingosine	Chemical		is linked to		possibly			cyclo-oxygenase pathway	Process				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_126_1_189_s_170	10051135	Therefore there appears to be a link between the sphingosine and cyclo-oxygenase pathways in the TNF-mediated coronary constriction, but the direct cardiac depressant actions of TNF are dependant on the conversion of ceramide of sphingosine, and do not involve the cyclo-oxygenase pathway.	transcription
78843	1	336019	6	NULL	NULL	0	NULL	TNF	GP		depresses					cardiac actions	Process				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_126_1_189_s_170	10051135	Therefore there appears to be a link between the sphingosine and cyclo-oxygenase pathways in the TNF-mediated coronary constriction, but the direct cardiac depressant actions of TNF are dependant on the conversion of ceramide of sphingosine, and do not involve the cyclo-oxygenase pathway.	transcription
78844	2	336019	6	NULL	NULL	0	NULL	statement 1	Process		does not involve					cyclo-oxygenase pathway	Process				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_126_1_189_s_170	10051135	Therefore there appears to be a link between the sphingosine and cyclo-oxygenase pathways in the TNF-mediated coronary constriction, but the direct cardiac depressant actions of TNF are dependant on the conversion of ceramide of sphingosine, and do not involve the cyclo-oxygenase pathway.	transcription
78845	3	336019	6	NULL	NULL	0	NULL	ceramide	Chemical		is converted to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_126_1_189_s_170	10051135	Therefore there appears to be a link between the sphingosine and cyclo-oxygenase pathways in the TNF-mediated coronary constriction, but the direct cardiac depressant actions of TNF are dependant on the conversion of ceramide of sphingosine, and do not involve the cyclo-oxygenase pathway.	transcription
78846	4	336019	6	NULL	NULL	0	NULL	statement 1	Process		is dependent on					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_126_1_189_s_170	10051135	Therefore there appears to be a link between the sphingosine and cyclo-oxygenase pathways in the TNF-mediated coronary constriction, but the direct cardiac depressant actions of TNF are dependant on the conversion of ceramide of sphingosine, and do not involve the cyclo-oxygenase pathway.	transcription
60111	1	336020	5	NULL	NULL	0	NULL	S1P	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_40_37323_s_254	12138095	Whereas S1P-induced apoptosis was caspase-dependent, the cytotoxic effect of sphingosine was caspase-independent, raising the possibility that sphingosine may trigger apoptosis via a caspase-independent release of apoptosis-inducing factor, as described for ceramide in lymphoid cells ( 31).	transcription
60112	2	336020	5	NULL	NULL	0	NULL	statement 1			is dependent on					caspase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_40_37323_s_254	12138095	Whereas S1P-induced apoptosis was caspase-dependent, the cytotoxic effect of sphingosine was caspase-independent, raising the possibility that sphingosine may trigger apoptosis via a caspase-independent release of apoptosis-inducing factor, as described for ceramide in lymphoid cells ( 31).	transcription
60113	3	336020	5	NULL	NULL	0	NULL	sphingosine	Chemical	cytotoxic effect of	is independent of					caspase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_40_37323_s_254	12138095	Whereas S1P-induced apoptosis was caspase-dependent, the cytotoxic effect of sphingosine was caspase-independent, raising the possibility that sphingosine may trigger apoptosis via a caspase-independent release of apoptosis-inducing factor, as described for ceramide in lymphoid cells ( 31).	transcription
60114	4	336020	5	NULL	NULL	0	NULL	sphingosine	Chemical		triggers		may			apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_40_37323_s_254	12138095	Whereas S1P-induced apoptosis was caspase-dependent, the cytotoxic effect of sphingosine was caspase-independent, raising the possibility that sphingosine may trigger apoptosis via a caspase-independent release of apoptosis-inducing factor, as described for ceramide in lymphoid cells ( 31).	transcription
60115	5	336020	5	NULL	NULL	0	NULL	apoptosis-inducing factor	Chemical	release of	is independent of					caspase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_40_37323_s_254	12138095	Whereas S1P-induced apoptosis was caspase-dependent, the cytotoxic effect of sphingosine was caspase-independent, raising the possibility that sphingosine may trigger apoptosis via a caspase-independent release of apoptosis-inducing factor, as described for ceramide in lymphoid cells ( 31).	transcription
60116	6	336020	5	NULL	NULL	0	NULL	statement 4	Process		via					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_40_37323_s_254	12138095	Whereas S1P-induced apoptosis was caspase-dependent, the cytotoxic effect of sphingosine was caspase-independent, raising the possibility that sphingosine may trigger apoptosis via a caspase-independent release of apoptosis-inducing factor, as described for ceramide in lymphoid cells ( 31).	transcription
60117	7	336020	5	NULL	NULL	0	NULL	ceramide	Chemical		triggers					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_40_37323_s_254	12138095	Whereas S1P-induced apoptosis was caspase-dependent, the cytotoxic effect of sphingosine was caspase-independent, raising the possibility that sphingosine may trigger apoptosis via a caspase-independent release of apoptosis-inducing factor, as described for ceramide in lymphoid cells ( 31).	transcription
60118	8	336020	5	NULL	NULL	0	NULL	statement 7	Process		via					statement 5	Process				NULL	lymphoid cells	0	NULL	NULL	NULL	gw60_jbiolchem_277_40_37323_s_254	12138095	Whereas S1P-induced apoptosis was caspase-dependent, the cytotoxic effect of sphingosine was caspase-independent, raising the possibility that sphingosine may trigger apoptosis via a caspase-independent release of apoptosis-inducing factor, as described for ceramide in lymphoid cells ( 31).	transcription
78839	1	336020	6	NULL	NULL	0	NULL	S1P	GP		induces					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_40_37323_s_254	12138095	Whereas S1P-induced apoptosis was caspase-dependent, the cytotoxic effect of sphingosine was caspase-independent, raising the possibility that sphingosine may trigger apoptosis via a caspase-independent release of apoptosis-inducing factor, as described for ceramide in lymphoid cells ( 31).	transcription
78840	2	336020	6	NULL	NULL	0	NULL	statement 1	Process		is dependent on					caspase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_40_37323_s_254	12138095	Whereas S1P-induced apoptosis was caspase-dependent, the cytotoxic effect of sphingosine was caspase-independent, raising the possibility that sphingosine may trigger apoptosis via a caspase-independent release of apoptosis-inducing factor, as described for ceramide in lymphoid cells ( 31).	transcription
78841	3	336020	6	NULL	NULL	0	NULL	sphingosine	Chemical		exhibits					cytotoxic effect	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_40_37323_s_254	12138095	Whereas S1P-induced apoptosis was caspase-dependent, the cytotoxic effect of sphingosine was caspase-independent, raising the possibility that sphingosine may trigger apoptosis via a caspase-independent release of apoptosis-inducing factor, as described for ceramide in lymphoid cells ( 31).	transcription
78842	4	336020	6	NULL	NULL	0	NULL	statement 3	Process		does not depend on					caspase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_40_37323_s_254	12138095	Whereas S1P-induced apoptosis was caspase-dependent, the cytotoxic effect of sphingosine was caspase-independent, raising the possibility that sphingosine may trigger apoptosis via a caspase-independent release of apoptosis-inducing factor, as described for ceramide in lymphoid cells ( 31).	transcription
60119	1	336021	5	NULL	NULL	0	NULL	TNF signaling	Process		via					sphingolipids	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_10_7996_s_19	11777919	TNF signaling via sphingolipids is exemplified by two distinct pathways: the formation of ceramide resulting from the activation of sphingomyelinase or  de novo synthesis and the production of sphingosine 1-phosphate (S1P) upon sphingosine kinase (SphK) activation.	transcription
60120	2	336021	5	NULL	NULL	0	NULL	sphingomyelinase	Chemical	activation of	results in					ceramide	Chemical	fomation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_10_7996_s_19	11777919	TNF signaling via sphingolipids is exemplified by two distinct pathways: the formation of ceramide resulting from the activation of sphingomyelinase or  de novo synthesis and the production of sphingosine 1-phosphate (S1P) upon sphingosine kinase (SphK) activation.	transcription
60121	3	336021	5	NULL	NULL	0	NULL	statement 2	Process		exemplifies					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_10_7996_s_19	11777919	TNF signaling via sphingolipids is exemplified by two distinct pathways: the formation of ceramide resulting from the activation of sphingomyelinase or  de novo synthesis and the production of sphingosine 1-phosphate (S1P) upon sphingosine kinase (SphK) activation.	transcription
60122	4	336021	5	NULL	NULL	0	NULL	SphK	GP	activation of	produce					S1P	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_10_7996_s_19	11777919	TNF signaling via sphingolipids is exemplified by two distinct pathways: the formation of ceramide resulting from the activation of sphingomyelinase or  de novo synthesis and the production of sphingosine 1-phosphate (S1P) upon sphingosine kinase (SphK) activation.	transcription
60123	5	336021	5	NULL	NULL	0	NULL	statement 4	Process		exemplifies					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_10_7996_s_19	11777919	TNF signaling via sphingolipids is exemplified by two distinct pathways: the formation of ceramide resulting from the activation of sphingomyelinase or  de novo synthesis and the production of sphingosine 1-phosphate (S1P) upon sphingosine kinase (SphK) activation.	transcription
60124	6	336021	5	NULL	NULL	0	NULL	SphK	GP		is					sphingosine kinase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_10_7996_s_19	11777919	TNF signaling via sphingolipids is exemplified by two distinct pathways: the formation of ceramide resulting from the activation of sphingomyelinase or  de novo synthesis and the production of sphingosine 1-phosphate (S1P) upon sphingosine kinase (SphK) activation.	transcription
60125	7	336021	5	NULL	NULL	0	NULL	S1P	Chemical		is					sphingosine 1-phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_10_7996_s_19	11777919	TNF signaling via sphingolipids is exemplified by two distinct pathways: the formation of ceramide resulting from the activation of sphingomyelinase or  de novo synthesis and the production of sphingosine 1-phosphate (S1P) upon sphingosine kinase (SphK) activation.	transcription
78835	1	336021	6	NULL	NULL	0	NULL	sphingomyelinase	GP	activation of	results in					ceramide	Chemical	formation of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_10_7996_s_19	11777919	TNF signaling via sphingolipids is exemplified by two distinct pathways: the formation of ceramide resulting from the activation of sphingomyelinase or  de novo synthesis and the production of sphingosine 1-phosphate (S1P) upon sphingosine kinase (SphK) activation.	transcription
78836	2	336021	6	NULL	NULL	0	NULL	S1P	Chemical		is					sphingosine 1-phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_10_7996_s_19	11777919	TNF signaling via sphingolipids is exemplified by two distinct pathways: the formation of ceramide resulting from the activation of sphingomyelinase or  de novo synthesis and the production of sphingosine 1-phosphate (S1P) upon sphingosine kinase (SphK) activation.	transcription
78837	3	336021	6	NULL	NULL	0	NULL	SphK	GP		is					sphingosine kinase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_10_7996_s_19	11777919	TNF signaling via sphingolipids is exemplified by two distinct pathways: the formation of ceramide resulting from the activation of sphingomyelinase or  de novo synthesis and the production of sphingosine 1-phosphate (S1P) upon sphingosine kinase (SphK) activation.	transcription
78838	4	336021	6	NULL	NULL	0	NULL	SphK	GP	activation of	results in					S1P	GP	production of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_10_7996_s_19	11777919	TNF signaling via sphingolipids is exemplified by two distinct pathways: the formation of ceramide resulting from the activation of sphingomyelinase or  de novo synthesis and the production of sphingosine 1-phosphate (S1P) upon sphingosine kinase (SphK) activation.	transcription
60126	1	336022	5	NULL	NULL	0	NULL	ceramide	Chemical	elevation of	is induced by					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_82	10747891	Moreover, a higher concentration of fumonisin B1 (100 muM) not only inhibited elevation of ceramide induced by 5 muM sphingosine by more than 70% after 5 h of treatment, it also markedly enhanced apoptosis induced by sphingosine.	transcription
60127	2	336022	5	NULL	NULL	0	NULL	fumonisin B1	Chemical		inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_82	10747891	Moreover, a higher concentration of fumonisin B1 (100 muM) not only inhibited elevation of ceramide induced by 5 muM sphingosine by more than 70% after 5 h of treatment, it also markedly enhanced apoptosis induced by sphingosine.	transcription
60128	3	336022	5	NULL	NULL	0	NULL	apoptosis	Process		is induced by					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_82	10747891	Moreover, a higher concentration of fumonisin B1 (100 muM) not only inhibited elevation of ceramide induced by 5 muM sphingosine by more than 70% after 5 h of treatment, it also markedly enhanced apoptosis induced by sphingosine.	transcription
60129	4	336022	5	NULL	NULL	0	NULL	fumonisin B1	Chemical		enhances		markedly			statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_82	10747891	Moreover, a higher concentration of fumonisin B1 (100 muM) not only inhibited elevation of ceramide induced by 5 muM sphingosine by more than 70% after 5 h of treatment, it also markedly enhanced apoptosis induced by sphingosine.	transcription
78832	1	336022	6	NULL	NULL	0	NULL	sphingosine	Chemical		induces					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_82	10747891	Moreover, a higher concentration of fumonisin B1 (100 muM) not only inhibited elevation of ceramide induced by 5 muM sphingosine by more than 70% after 5 h of treatment, it also markedly enhanced apoptosis induced by sphingosine.	transcription
78833	2	336022	6	NULL	NULL	0	NULL	fumonisin B1 	Chemical		inhibits					ceramide	Chemical	elevation of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_82	10747891	Moreover, a higher concentration of fumonisin B1 (100 muM) not only inhibited elevation of ceramide induced by 5 muM sphingosine by more than 70% after 5 h of treatment, it also markedly enhanced apoptosis induced by sphingosine.	transcription
78834	3	336022	6	NULL	NULL	0	NULL	sphingosine	Chemical		induces					ceramide	Chemical	elevation of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_82	10747891	Moreover, a higher concentration of fumonisin B1 (100 muM) not only inhibited elevation of ceramide induced by 5 muM sphingosine by more than 70% after 5 h of treatment, it also markedly enhanced apoptosis induced by sphingosine.	transcription
60130	1	336023	5	NULL	NULL	0	NULL	sphingosine	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_266	10747891	Herein, we suggest that sphingosine, as well as ceramide, induces apoptosis in a mitochondria-dependent fashion, as Bcl-xL completely abolishes apoptosis, DEVDase activity, and release of cyt  c induced by C2-ceramide or by sphingosine.	transcription
60131	2	336023	5	NULL	NULL	0	NULL	statement 1	Process		is dependent on					mitochondria	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_266	10747891	Herein, we suggest that sphingosine, as well as ceramide, induces apoptosis in a mitochondria-dependent fashion, as Bcl-xL completely abolishes apoptosis, DEVDase activity, and release of cyt  c induced by C2-ceramide or by sphingosine.	transcription
60132	3	336023	5	NULL	NULL	0	NULL	sphingosine	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_266	10747891	Herein, we suggest that sphingosine, as well as ceramide, induces apoptosis in a mitochondria-dependent fashion, as Bcl-xL completely abolishes apoptosis, DEVDase activity, and release of cyt  c induced by C2-ceramide or by sphingosine.	transcription
60133	4	336023	5	NULL	NULL	0	NULL	statement 3	Process		is dependent on					mitochondria	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_266	10747891	Herein, we suggest that sphingosine, as well as ceramide, induces apoptosis in a mitochondria-dependent fashion, as Bcl-xL completely abolishes apoptosis, DEVDase activity, and release of cyt  c induced by C2-ceramide or by sphingosine.	transcription
60134	5	336023	5	NULL	NULL	0	NULL	Bcl-xL	GP		abolishes		completely			apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_266	10747891	Herein, we suggest that sphingosine, as well as ceramide, induces apoptosis in a mitochondria-dependent fashion, as Bcl-xL completely abolishes apoptosis, DEVDase activity, and release of cyt  c induced by C2-ceramide or by sphingosine.	transcription
60135	6	336023	5	NULL	NULL	0	NULL	Bcl-xL	GP		abolishes		completely			DEVDase	GP	activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_266	10747891	Herein, we suggest that sphingosine, as well as ceramide, induces apoptosis in a mitochondria-dependent fashion, as Bcl-xL completely abolishes apoptosis, DEVDase activity, and release of cyt  c induced by C2-ceramide or by sphingosine.	transcription
60136	7	336023	5	NULL	NULL	0	NULL	cyt c	GP	release of	is induced by					C2-ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_266	10747891	Herein, we suggest that sphingosine, as well as ceramide, induces apoptosis in a mitochondria-dependent fashion, as Bcl-xL completely abolishes apoptosis, DEVDase activity, and release of cyt  c induced by C2-ceramide or by sphingosine.	transcription
60137	8	336023	5	NULL	NULL	0	NULL	cyt c	GP	release of	is induced by					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_266	10747891	Herein, we suggest that sphingosine, as well as ceramide, induces apoptosis in a mitochondria-dependent fashion, as Bcl-xL completely abolishes apoptosis, DEVDase activity, and release of cyt  c induced by C2-ceramide or by sphingosine.	transcription
60138	9	336023	5	NULL	NULL	0	NULL	statement 7	Process		is an alternative to					statement 8	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_266	10747891	Herein, we suggest that sphingosine, as well as ceramide, induces apoptosis in a mitochondria-dependent fashion, as Bcl-xL completely abolishes apoptosis, DEVDase activity, and release of cyt  c induced by C2-ceramide or by sphingosine.	transcription
60139	10	336023	5	NULL	NULL	0	NULL	Bcl-xL	GP		abolishes		completely			statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_266	10747891	Herein, we suggest that sphingosine, as well as ceramide, induces apoptosis in a mitochondria-dependent fashion, as Bcl-xL completely abolishes apoptosis, DEVDase activity, and release of cyt  c induced by C2-ceramide or by sphingosine.	transcription
60140	11	336023	5	NULL	NULL	0	NULL	Bcl-xL	GP		abolishes		completely			statement 8	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_266	10747891	Herein, we suggest that sphingosine, as well as ceramide, induces apoptosis in a mitochondria-dependent fashion, as Bcl-xL completely abolishes apoptosis, DEVDase activity, and release of cyt  c induced by C2-ceramide or by sphingosine.	transcription
66669	1	336023	7	NULL	NULL	0	NULL	sphingosine	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_266	10747891	Herein, we suggest that sphingosine, as well as ceramide, induces apoptosis in a mitochondria-dependent fashion, as Bcl-xL completely abolishes apoptosis, DEVDase activity, and release of cyt  c induced by C2-ceramide or by sphingosine.	transcription
66670	2	336023	7	NULL	NULL	0	NULL	ceramide	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_266	10747891	Herein, we suggest that sphingosine, as well as ceramide, induces apoptosis in a mitochondria-dependent fashion, as Bcl-xL completely abolishes apoptosis, DEVDase activity, and release of cyt  c induced by C2-ceramide or by sphingosine.	transcription
66671	3	336023	7	NULL	NULL	0	NULL	statement 1	Process		depends on					mitochondria	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_266	10747891	Herein, we suggest that sphingosine, as well as ceramide, induces apoptosis in a mitochondria-dependent fashion, as Bcl-xL completely abolishes apoptosis, DEVDase activity, and release of cyt  c induced by C2-ceramide or by sphingosine.	transcription
66672	4	336023	7	NULL	NULL	0	NULL	statement 2	Process		depends on					mitochondria	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_266	10747891	Herein, we suggest that sphingosine, as well as ceramide, induces apoptosis in a mitochondria-dependent fashion, as Bcl-xL completely abolishes apoptosis, DEVDase activity, and release of cyt  c induced by C2-ceramide or by sphingosine.	transcription
66673	5	336023	7	NULL	NULL	0	NULL	Bcl-xL	GP		abolishes		completely			apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_266	10747891	Herein, we suggest that sphingosine, as well as ceramide, induces apoptosis in a mitochondria-dependent fashion, as Bcl-xL completely abolishes apoptosis, DEVDase activity, and release of cyt  c induced by C2-ceramide or by sphingosine.	transcription
66674	6	336023	7	NULL	NULL	0	NULL	Bcl-xL	GP		abolishes		completely			DEVDase	GP	activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_266	10747891	Herein, we suggest that sphingosine, as well as ceramide, induces apoptosis in a mitochondria-dependent fashion, as Bcl-xL completely abolishes apoptosis, DEVDase activity, and release of cyt  c induced by C2-ceramide or by sphingosine.	transcription
66675	7	336023	7	NULL	NULL	0	NULL	 C2-ceramide	Chemical		induce					cyt c	GP	release of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_266	10747891	Herein, we suggest that sphingosine, as well as ceramide, induces apoptosis in a mitochondria-dependent fashion, as Bcl-xL completely abolishes apoptosis, DEVDase activity, and release of cyt  c induced by C2-ceramide or by sphingosine.	transcription
66676	8	336023	7	NULL	NULL	NULL	NULL	sphingosine	Chemical		induce					cyt c	GP	release of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_266	10747891	Herein, we suggest that sphingosine, as well as ceramide, induces apoptosis in a mitochondria-dependent fashion, as Bcl-xL completely abolishes apoptosis, DEVDase activity, and release of cyt  c induced by C2-ceramide or by sphingosine.	transcription
66677	9	336023	7	NULL	NULL	0	NULL	statement 7	Process		is an alternative to					statement 8	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_266	10747891	Herein, we suggest that sphingosine, as well as ceramide, induces apoptosis in a mitochondria-dependent fashion, as Bcl-xL completely abolishes apoptosis, DEVDase activity, and release of cyt  c induced by C2-ceramide or by sphingosine.	transcription
66678	10	336023	7	NULL	NULL	0	NULL	Bcl-xL	GP		abolishes		completely			statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_266	10747891	Herein, we suggest that sphingosine, as well as ceramide, induces apoptosis in a mitochondria-dependent fashion, as Bcl-xL completely abolishes apoptosis, DEVDase activity, and release of cyt  c induced by C2-ceramide or by sphingosine.	transcription
66679	11	336023	7	NULL	NULL	0	NULL	Bcl-xL	GP		abolishes		completely			statement 8	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_266	10747891	Herein, we suggest that sphingosine, as well as ceramide, induces apoptosis in a mitochondria-dependent fashion, as Bcl-xL completely abolishes apoptosis, DEVDase activity, and release of cyt  c induced by C2-ceramide or by sphingosine.	transcription
60141	1	336024	5	NULL	NULL	0	NULL	sphingosine	Chemical		increases					Ca2+	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_19_11148_s_10	8626660	Sphingosine,  stearylamine, and psychosine increased  [Ca ]   and  diacylglycerol (DG) kinase activation; however, ceramide did not,  whereas sphingosine 1-phosphate slightly activated DG kinase without  elevation of [Ca ] .	transcription
60142	2	336024	5	NULL	NULL	0	NULL	sphingosine	Chemical		increases					DG kinase	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_19_11148_s_10	8626660	Sphingosine,  stearylamine, and psychosine increased  [Ca ]   and  diacylglycerol (DG) kinase activation; however, ceramide did not,  whereas sphingosine 1-phosphate slightly activated DG kinase without  elevation of [Ca ] .	transcription
60143	3	336024	5	NULL	NULL	0	NULL	stearylamine	Chemical		increases					Ca2+	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_19_11148_s_10	8626660	Sphingosine,  stearylamine, and psychosine increased  [Ca ]   and  diacylglycerol (DG) kinase activation; however, ceramide did not,  whereas sphingosine 1-phosphate slightly activated DG kinase without  elevation of [Ca ] .	transcription
60144	4	336024	5	NULL	NULL	0	NULL	stearylamine	Chemical		increases					DG kinase	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_19_11148_s_10	8626660	Sphingosine,  stearylamine, and psychosine increased  [Ca ]   and  diacylglycerol (DG) kinase activation; however, ceramide did not,  whereas sphingosine 1-phosphate slightly activated DG kinase without  elevation of [Ca ] .	transcription
60145	5	336024	5	NULL	NULL	0	NULL	psychosine	Chemical		increases					Ca2+	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_19_11148_s_10	8626660	Sphingosine,  stearylamine, and psychosine increased  [Ca ]   and  diacylglycerol (DG) kinase activation; however, ceramide did not,  whereas sphingosine 1-phosphate slightly activated DG kinase without  elevation of [Ca ] .	transcription
60146	6	336024	5	NULL	NULL	0	NULL	psychosine	Chemical		increases					DG kinase	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_19_11148_s_10	8626660	Sphingosine,  stearylamine, and psychosine increased  [Ca ]   and  diacylglycerol (DG) kinase activation; however, ceramide did not,  whereas sphingosine 1-phosphate slightly activated DG kinase without  elevation of [Ca ] .	transcription
60147	7	336024	5	NULL	NULL	0	NULL	DG kinase	GP		is					diacylglycerol kinase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_19_11148_s_10	8626660	Sphingosine,  stearylamine, and psychosine increased  [Ca ]   and  diacylglycerol (DG) kinase activation; however, ceramide did not,  whereas sphingosine 1-phosphate slightly activated DG kinase without  elevation of [Ca ] .	transcription
60148	8	336024	5	NULL	NULL	0	NULL	ceramide	Chemical		does not increase					Ca2+	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_19_11148_s_10	8626660	Sphingosine,  stearylamine, and psychosine increased  [Ca ]   and  diacylglycerol (DG) kinase activation; however, ceramide did not,  whereas sphingosine 1-phosphate slightly activated DG kinase without  elevation of [Ca ] .	transcription
60149	9	336024	5	NULL	NULL	0	NULL	ceramide	Chemical		does not increase					DG kinase	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_19_11148_s_10	8626660	Sphingosine,  stearylamine, and psychosine increased  [Ca ]   and  diacylglycerol (DG) kinase activation; however, ceramide did not,  whereas sphingosine 1-phosphate slightly activated DG kinase without  elevation of [Ca ] .	transcription
60150	10	336024	5	NULL	NULL	0	NULL	sphingosine 1-phosphate	Chemical		activates		slightly			DG kinase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_19_11148_s_10	8626660	Sphingosine,  stearylamine, and psychosine increased  [Ca ]   and  diacylglycerol (DG) kinase activation; however, ceramide did not,  whereas sphingosine 1-phosphate slightly activated DG kinase without  elevation of [Ca ] .	transcription
60151	11	336024	5	NULL	NULL	0	NULL	statement 10	Process		occurs without elevation of					Ca2+	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_19_11148_s_10	8626660	Sphingosine,  stearylamine, and psychosine increased  [Ca ]   and  diacylglycerol (DG) kinase activation; however, ceramide did not,  whereas sphingosine 1-phosphate slightly activated DG kinase without  elevation of [Ca ] .	transcription
66680	1	336024	7	NULL	NULL	0	NULL	Sphingosine	Chemical		increase					Ca	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_19_11148_s_10	8626660	Sphingosine,  stearylamine, and psychosine increased  [Ca ]   and  diacylglycerol (DG) kinase activation; however, ceramide did not,  whereas sphingosine 1-phosphate slightly activated DG kinase without  elevation of [Ca ] .	transcription
66681	2	336024	7	NULL	NULL	0	NULL	stearylamine	Chemical		increase					Ca	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_19_11148_s_10	8626660	Sphingosine,  stearylamine, and psychosine increased  [Ca ]   and  diacylglycerol (DG) kinase activation; however, ceramide did not,  whereas sphingosine 1-phosphate slightly activated DG kinase without  elevation of [Ca ] .	transcription
66682	3	336024	7	NULL	NULL	NULL	NULL	psychosine	Chemical		increase					Ca	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_19_11148_s_10	8626660	Sphingosine,  stearylamine, and psychosine increased  [Ca ]   and  diacylglycerol (DG) kinase activation; however, ceramide did not,  whereas sphingosine 1-phosphate slightly activated DG kinase without  elevation of [Ca ] .	transcription
66683	4	336024	7	NULL	NULL	0	NULL	Sphingosine	Chemical		increase					DG kinase	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_19_11148_s_10	8626660	Sphingosine,  stearylamine, and psychosine increased  [Ca ]   and  diacylglycerol (DG) kinase activation; however, ceramide did not,  whereas sphingosine 1-phosphate slightly activated DG kinase without  elevation of [Ca ] .	transcription
66684	5	336024	7	NULL	NULL	0	NULL	stearylamine	Chemical		increase					DG kinase	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_19_11148_s_10	8626660	Sphingosine,  stearylamine, and psychosine increased  [Ca ]   and  diacylglycerol (DG) kinase activation; however, ceramide did not,  whereas sphingosine 1-phosphate slightly activated DG kinase without  elevation of [Ca ] .	transcription
66685	6	336024	7	NULL	NULL	0	NULL	psychosine	Chemical		increase					DG kinase	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_19_11148_s_10	8626660	Sphingosine,  stearylamine, and psychosine increased  [Ca ]   and  diacylglycerol (DG) kinase activation; however, ceramide did not,  whereas sphingosine 1-phosphate slightly activated DG kinase without  elevation of [Ca ] .	transcription
66686	7	336024	7	NULL	NULL	NULL	NULL	ceramide	Chemical		does not activate					DG kinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_19_11148_s_10	8626660	Sphingosine,  stearylamine, and psychosine increased  [Ca ]   and  diacylglycerol (DG) kinase activation; however, ceramide did not,  whereas sphingosine 1-phosphate slightly activated DG kinase without  elevation of [Ca ] .	transcription
66687	8	336024	7	NULL	NULL	0	NULL	sphingosine 1-phosphate	Chemical		activates		slightly			DG kinase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_19_11148_s_10	8626660	Sphingosine,  stearylamine, and psychosine increased  [Ca ]   and  diacylglycerol (DG) kinase activation; however, ceramide did not,  whereas sphingosine 1-phosphate slightly activated DG kinase without  elevation of [Ca ] .	transcription
66688	9	336024	7	NULL	NULL	0	NULL	statement 8	Process		occur without					Ca	Chemical	elevation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_19_11148_s_10	8626660	Sphingosine,  stearylamine, and psychosine increased  [Ca ]   and  diacylglycerol (DG) kinase activation; however, ceramide did not,  whereas sphingosine 1-phosphate slightly activated DG kinase without  elevation of [Ca ] .	transcription
66689	10	336024	7	NULL	NULL	0	NULL	DG	Chemical		is					diacylglycerol	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_19_11148_s_10	8626660	Sphingosine,  stearylamine, and psychosine increased  [Ca ]   and  diacylglycerol (DG) kinase activation; however, ceramide did not,  whereas sphingosine 1-phosphate slightly activated DG kinase without  elevation of [Ca ] .	transcription
60170	1	336025	5	NULL	NULL	0	NULL	ceramide	Chemical		is formed from		directly			sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_21_12646_s_269	8647877	The inhibitor can also be used to distinguish  those effects of sphingosine that are mediated through the direct  formation of ceramide from sphingosine since those effects would be  anticipated to be inhibitable by fumonisin B1.	transcription
66690	1	336025	7	NULL	NULL	0	NULL	ceramide	Chemical		formed from					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_21_12646_s_269	8647877	The inhibitor can also be used to distinguish  those effects of sphingosine that are mediated through the direct  formation of ceramide from sphingosine since those effects would be  anticipated to be inhibitable by fumonisin B1.	transcription
66691	2	336025	7	NULL	NULL	0	NULL	fumonisin B1	Chemical		inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_21_12646_s_269	8647877	The inhibitor can also be used to distinguish  those effects of sphingosine that are mediated through the direct  formation of ceramide from sphingosine since those effects would be  anticipated to be inhibitable by fumonisin B1.	transcription
60171	1	336026	5	NULL	NULL	0	NULL	sphingosine	Chemical		does not inhibit					PLD	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_40_24800_s_155	8798752	It is unlikely that ceramide acts via its metabolism to sphingosine since our intact cell data demonstrate that sphingosine does not inhibit PLD as potently as C6-ceramide, and in the cell-free assay, no preincubation is necessary for maximal effect.	transcription
60172	2	336026	5	NULL	NULL	0	NULL	C6-ceramide	Chemical		does not inhibit					PLD	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_40_24800_s_155	8798752	It is unlikely that ceramide acts via its metabolism to sphingosine since our intact cell data demonstrate that sphingosine does not inhibit PLD as potently as C6-ceramide, and in the cell-free assay, no preincubation is necessary for maximal effect.	transcription
60173	3	336026	5	NULL	NULL	0	NULL	statement 1	Process		not as potent as					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_40_24800_s_155	8798752	It is unlikely that ceramide acts via its metabolism to sphingosine since our intact cell data demonstrate that sphingosine does not inhibit PLD as potently as C6-ceramide, and in the cell-free assay, no preincubation is necessary for maximal effect.	transcription
66692	1	336026	7	NULL	NULL	0	NULL	sphingosine	Chemical		does not inhibit					PLD	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_40_24800_s_155	8798752	It is unlikely that ceramide acts via its metabolism to sphingosine since our intact cell data demonstrate that sphingosine does not inhibit PLD as potently as C6-ceramide, and in the cell-free assay, no preincubation is necessary for maximal effect.	transcription
66693	2	336026	7	NULL	NULL	0	NULL	C6-ceramide	Chemical		does not inhibit					PLD	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_40_24800_s_155	8798752	It is unlikely that ceramide acts via its metabolism to sphingosine since our intact cell data demonstrate that sphingosine does not inhibit PLD as potently as C6-ceramide, and in the cell-free assay, no preincubation is necessary for maximal effect.	transcription
66694	3	336026	7	NULL	NULL	0	NULL	statement 1	Process		is not as potent as					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_40_24800_s_155	8798752	It is unlikely that ceramide acts via its metabolism to sphingosine since our intact cell data demonstrate that sphingosine does not inhibit PLD as potently as C6-ceramide, and in the cell-free assay, no preincubation is necessary for maximal effect.	transcription
60174	1	336027	5	NULL	NULL	0	NULL	SPT	GP		is					serine palmitoyltransferase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_49_32487_s_28	9829981	The first step in the pathway involves serine palmitoyltransferase (SPT), the enzyme that catalyzes the condensation of palmitoyl-CoA and serine to form dehydrosphinganine, a precursor of sphingosine ( 9,  10); sphingosine is then acylated to form ceramide ( 11,  12).	transcription
60175	2	336027	5	NULL	NULL	0	NULL	palmitoyl-CoA	Chemical		is condensed to					dehydrosphinganine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_49_32487_s_28	9829981	The first step in the pathway involves serine palmitoyltransferase (SPT), the enzyme that catalyzes the condensation of palmitoyl-CoA and serine to form dehydrosphinganine, a precursor of sphingosine ( 9,  10); sphingosine is then acylated to form ceramide ( 11,  12).	transcription
60176	3	336027	5	NULL	NULL	0	NULL	serine	AminoAcid		is condensed to					dehydrosphinganine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_49_32487_s_28	9829981	The first step in the pathway involves serine palmitoyltransferase (SPT), the enzyme that catalyzes the condensation of palmitoyl-CoA and serine to form dehydrosphinganine, a precursor of sphingosine ( 9,  10); sphingosine is then acylated to form ceramide ( 11,  12).	transcription
60177	4	336027	5	NULL	NULL	0	NULL	SPT	GP		catalyzes					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_49_32487_s_28	9829981	The first step in the pathway involves serine palmitoyltransferase (SPT), the enzyme that catalyzes the condensation of palmitoyl-CoA and serine to form dehydrosphinganine, a precursor of sphingosine ( 9,  10); sphingosine is then acylated to form ceramide ( 11,  12).	transcription
60178	5	336027	5	NULL	NULL	0	NULL	SPT	GP		catalyzes					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_49_32487_s_28	9829981	The first step in the pathway involves serine palmitoyltransferase (SPT), the enzyme that catalyzes the condensation of palmitoyl-CoA and serine to form dehydrosphinganine, a precursor of sphingosine ( 9,  10); sphingosine is then acylated to form ceramide ( 11,  12).	transcription
60179	6	336027	5	NULL	NULL	0	NULL	dehydrosphinganine	Chemical		is a precursor of					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_49_32487_s_28	9829981	The first step in the pathway involves serine palmitoyltransferase (SPT), the enzyme that catalyzes the condensation of palmitoyl-CoA and serine to form dehydrosphinganine, a precursor of sphingosine ( 9,  10); sphingosine is then acylated to form ceramide ( 11,  12).	transcription
60180	7	336027	5	NULL	NULL	0	NULL	sphingosine	Chemical		acylated to					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_49_32487_s_28	9829981	The first step in the pathway involves serine palmitoyltransferase (SPT), the enzyme that catalyzes the condensation of palmitoyl-CoA and serine to form dehydrosphinganine, a precursor of sphingosine ( 9,  10); sphingosine is then acylated to form ceramide ( 11,  12).	transcription
66695	1	336027	7	NULL	NULL	0	NULL	palmitoyl-CoA	Chemical		condense to form					dehydrosphinganine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_49_32487_s_28	9829981	The first step in the pathway involves serine palmitoyltransferase (SPT), the enzyme that catalyzes the condensation of palmitoyl-CoA and serine to form dehydrosphinganine, a precursor of sphingosine ( 9,  10); sphingosine is then acylated to form ceramide ( 11,  12).	transcription
66696	2	336027	7	NULL	NULL	0	NULL	serine	AminoAcid		condense to form					dehydrosphinganine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_49_32487_s_28	9829981	The first step in the pathway involves serine palmitoyltransferase (SPT), the enzyme that catalyzes the condensation of palmitoyl-CoA and serine to form dehydrosphinganine, a precursor of sphingosine ( 9,  10); sphingosine is then acylated to form ceramide ( 11,  12).	transcription
66697	3	336027	7	NULL	NULL	0	NULL	statement 1	Process		occur along with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_49_32487_s_28	9829981	The first step in the pathway involves serine palmitoyltransferase (SPT), the enzyme that catalyzes the condensation of palmitoyl-CoA and serine to form dehydrosphinganine, a precursor of sphingosine ( 9,  10); sphingosine is then acylated to form ceramide ( 11,  12).	transcription
66698	4	336027	7	NULL	NULL	0	NULL	SPT	GP		catalyze					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_49_32487_s_28	9829981	The first step in the pathway involves serine palmitoyltransferase (SPT), the enzyme that catalyzes the condensation of palmitoyl-CoA and serine to form dehydrosphinganine, a precursor of sphingosine ( 9,  10); sphingosine is then acylated to form ceramide ( 11,  12).	transcription
66699	5	336027	7	NULL	NULL	0	NULL	dehydrosphinganine	Chemical		is a precursor of					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_49_32487_s_28	9829981	The first step in the pathway involves serine palmitoyltransferase (SPT), the enzyme that catalyzes the condensation of palmitoyl-CoA and serine to form dehydrosphinganine, a precursor of sphingosine ( 9,  10); sphingosine is then acylated to form ceramide ( 11,  12).	transcription
66700	6	336027	7	NULL	NULL	0	NULL	sphingosine	Chemical		undergoes					acylation	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_49_32487_s_28	9829981	The first step in the pathway involves serine palmitoyltransferase (SPT), the enzyme that catalyzes the condensation of palmitoyl-CoA and serine to form dehydrosphinganine, a precursor of sphingosine ( 9,  10); sphingosine is then acylated to form ceramide ( 11,  12).	transcription
66701	7	336027	7	NULL	NULL	0	NULL	statement 6	Process		leads to					ceramide	Chemical	formation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_49_32487_s_28	9829981	The first step in the pathway involves serine palmitoyltransferase (SPT), the enzyme that catalyzes the condensation of palmitoyl-CoA and serine to form dehydrosphinganine, a precursor of sphingosine ( 9,  10); sphingosine is then acylated to form ceramide ( 11,  12).	transcription
66702	8	336027	7	NULL	NULL	0	NULL	SPT	GP		is					serine palmitoyltransferase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_49_32487_s_28	9829981	The first step in the pathway involves serine palmitoyltransferase (SPT), the enzyme that catalyzes the condensation of palmitoyl-CoA and serine to form dehydrosphinganine, a precursor of sphingosine ( 9,  10); sphingosine is then acylated to form ceramide ( 11,  12).	transcription
60181	1	336028	5	NULL	NULL	0	NULL	SPP	Chemical		is a metabolite of					ceramide	Chemical				NULL	PC12 cells	NULL	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_176	9278531	In this study, we found that in PC12 cells NGF stimulated the formation of a further metabolite of ceramide, SPP, by markedly activating sphingosine kinase, the enzyme that catalyzes the phosphorylation of sphingosine to SPP.	transcription
60182	2	336028	5	NULL	NULL	0	NULL	sphingosine	Chemical		is phosphorylated to					SPP	Chemical				NULL	PC12 cells	NULL	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_176	9278531	In this study, we found that in PC12 cells NGF stimulated the formation of a further metabolite of ceramide, SPP, by markedly activating sphingosine kinase, the enzyme that catalyzes the phosphorylation of sphingosine to SPP.	transcription
60183	3	336028	5	NULL	NULL	0	NULL	sphingosine kinase	GP	activated	catalyzes					statement 2	Process				NULL	PC12 cells	NULL	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_176	9278531	In this study, we found that in PC12 cells NGF stimulated the formation of a further metabolite of ceramide, SPP, by markedly activating sphingosine kinase, the enzyme that catalyzes the phosphorylation of sphingosine to SPP.	transcription
60184	4	336028	5	NULL	NULL	0	NULL	NGF	GP		activates		markedly			sphingosine kinase	GP				NULL	PC12 cells	NULL	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_176	9278531	In this study, we found that in PC12 cells NGF stimulated the formation of a further metabolite of ceramide, SPP, by markedly activating sphingosine kinase, the enzyme that catalyzes the phosphorylation of sphingosine to SPP.	transcription
60185	5	336028	5	NULL	NULL	0	NULL	statement 4	Process		leads to					statement 3	Process				NULL	PC12 cells	NULL	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_176	9278531	In this study, we found that in PC12 cells NGF stimulated the formation of a further metabolite of ceramide, SPP, by markedly activating sphingosine kinase, the enzyme that catalyzes the phosphorylation of sphingosine to SPP.	transcription
60186	6	336028	5	NULL	NULL	0	NULL	NGF	GP		stimulates					SPP	Chemical	fomation of			NULL	PC12 cells	0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_176	9278531	In this study, we found that in PC12 cells NGF stimulated the formation of a further metabolite of ceramide, SPP, by markedly activating sphingosine kinase, the enzyme that catalyzes the phosphorylation of sphingosine to SPP.	transcription
66703	1	336028	7	NULL	NULL	0	NULL	NGF	GP		stimulate					SPP	Chemical	formation of			NULL	PC12 cells	0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_176	9278531	In this study, we found that in PC12 cells NGF stimulated the formation of a further metabolite of ceramide, SPP, by markedly activating sphingosine kinase, the enzyme that catalyzes the phosphorylation of sphingosine to SPP.	transcription
66704	2	336028	7	NULL	NULL	0	NULL	statement 1	Process		occur by					sphingosine kinase	GP	activating			NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_176	9278531	In this study, we found that in PC12 cells NGF stimulated the formation of a further metabolite of ceramide, SPP, by markedly activating sphingosine kinase, the enzyme that catalyzes the phosphorylation of sphingosine to SPP.	transcription
66705	3	336028	7	NULL	NULL	0	NULL	sphingosine	Chemical		phosphorylated to					SPP	Chemical				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_176	9278531	In this study, we found that in PC12 cells NGF stimulated the formation of a further metabolite of ceramide, SPP, by markedly activating sphingosine kinase, the enzyme that catalyzes the phosphorylation of sphingosine to SPP.	transcription
66706	4	336028	7	NULL	NULL	0	NULL	sphingosine kinase	GP		catalyze					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_176	9278531	In this study, we found that in PC12 cells NGF stimulated the formation of a further metabolite of ceramide, SPP, by markedly activating sphingosine kinase, the enzyme that catalyzes the phosphorylation of sphingosine to SPP.	transcription
60187	1	336029	5	NULL	NULL	0	NULL	PLD	GP		is activated by					ET-1	GP				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_292_2_629_s_9	10640300	Inhibition by genistein and D-erythro- N-hexanoyl-sphingosine was additive, whereas inhibition by Ro-31-8220 and D-erythro- N-hexanoyl-sphingosine was not, indicating that ceramide affected the PKC-dependent process involved in PLD activation by ET-1.	transcription
60188	2	336029	5	NULL	NULL	0	NULL	statement 1	Process		is dependent on					PKC	GP				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_292_2_629_s_9	10640300	Inhibition by genistein and D-erythro- N-hexanoyl-sphingosine was additive, whereas inhibition by Ro-31-8220 and D-erythro- N-hexanoyl-sphingosine was not, indicating that ceramide affected the PKC-dependent process involved in PLD activation by ET-1.	transcription
60189	3	336029	5	NULL	NULL	0	NULL	ceramide	Chemical		affects					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_292_2_629_s_9	10640300	Inhibition by genistein and D-erythro- N-hexanoyl-sphingosine was additive, whereas inhibition by Ro-31-8220 and D-erythro- N-hexanoyl-sphingosine was not, indicating that ceramide affected the PKC-dependent process involved in PLD activation by ET-1.	transcription
66707	1	336029	7	NULL	NULL	0	NULL	ET-1	GP		activate					PLD	GP				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_292_2_629_s_9	10640300	Inhibition by genistein and D-erythro- N-hexanoyl-sphingosine was additive, whereas inhibition by Ro-31-8220 and D-erythro- N-hexanoyl-sphingosine was not, indicating that ceramide affected the PKC-dependent process involved in PLD activation by ET-1.	transcription
66708	2	336029	7	NULL	NULL	0	NULL	ceramide	Chemical		affects					PKC-dependent process	Process				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_292_2_629_s_9	10640300	Inhibition by genistein and D-erythro- N-hexanoyl-sphingosine was additive, whereas inhibition by Ro-31-8220 and D-erythro- N-hexanoyl-sphingosine was not, indicating that ceramide affected the PKC-dependent process involved in PLD activation by ET-1.	transcription
66709	3	336029	7	NULL	NULL	0	NULL	PKC-dependent process	Process		involved in					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_292_2_629_s_9	10640300	Inhibition by genistein and D-erythro- N-hexanoyl-sphingosine was additive, whereas inhibition by Ro-31-8220 and D-erythro- N-hexanoyl-sphingosine was not, indicating that ceramide affected the PKC-dependent process involved in PLD activation by ET-1.	transcription
60190	1	336030	5	NULL	NULL	0	NULL	D- erythro-sphingosine, N-acetyl-(C2-ceramides) 1	Chemical		is a type of					cell-permeant ceramide	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_48_47498_s_14	12952965	By stimulating NHEK with cell-permeant ceramides ( e.g.D- erythro-sphingosine,  N-acetyl-(C2-ceramides)  1 or D-erythrosphingosine,  N-hexanoyl-(C6-ceramides)) it has recently been observed that ceramide-induced expression of the human ICAM-1 gene is mediated through activation of AP-2, indicating that ceramides are capable of activating transcription factors in human cells through a yet unknown mechanism ( ).	transcription
60191	2	336030	5	NULL	NULL	0	NULL	D-erythrosphingosine, N-hexanoyl-(C6-ceramides)	Chemical		is a type of					cell-permeant ceramide	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_48_47498_s_14	12952965	By stimulating NHEK with cell-permeant ceramides ( e.g.D- erythro-sphingosine,  N-acetyl-(C2-ceramides)  1 or D-erythrosphingosine,  N-hexanoyl-(C6-ceramides)) it has recently been observed that ceramide-induced expression of the human ICAM-1 gene is mediated through activation of AP-2, indicating that ceramides are capable of activating transcription factors in human cells through a yet unknown mechanism ( ).	transcription
60192	3	336030	5	NULL	NULL	0	NULL	D-erythrosphingosine, N-hexanoyl-(C6-ceramides)	Chemical		stimulates					NHEK	Cell				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_48_47498_s_14	12952965	By stimulating NHEK with cell-permeant ceramides ( e.g.D- erythro-sphingosine,  N-acetyl-(C2-ceramides)  1 or D-erythrosphingosine,  N-hexanoyl-(C6-ceramides)) it has recently been observed that ceramide-induced expression of the human ICAM-1 gene is mediated through activation of AP-2, indicating that ceramides are capable of activating transcription factors in human cells through a yet unknown mechanism ( ).	transcription
60193	4	336030	5	NULL	NULL	0	NULL	D- erythro-sphingosine, N-acetyl-(C2-ceramides) 1	Chemical		stimulates					NHEK	Cell				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_48_47498_s_14	12952965	By stimulating NHEK with cell-permeant ceramides ( e.g.D- erythro-sphingosine,  N-acetyl-(C2-ceramides)  1 or D-erythrosphingosine,  N-hexanoyl-(C6-ceramides)) it has recently been observed that ceramide-induced expression of the human ICAM-1 gene is mediated through activation of AP-2, indicating that ceramides are capable of activating transcription factors in human cells through a yet unknown mechanism ( ).	transcription
60194	5	336030	5	NULL	NULL	0	NULL	ceramide	Chemical		induce					ICAM-1 gene	GP	expression of;;human			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_48_47498_s_14	12952965	By stimulating NHEK with cell-permeant ceramides ( e.g.D- erythro-sphingosine,  N-acetyl-(C2-ceramides)  1 or D-erythrosphingosine,  N-hexanoyl-(C6-ceramides)) it has recently been observed that ceramide-induced expression of the human ICAM-1 gene is mediated through activation of AP-2, indicating that ceramides are capable of activating transcription factors in human cells through a yet unknown mechanism ( ).	transcription
60195	6	336030	5	NULL	NULL	0	NULL	statement 5	Process		is mediated through					AP-2	GP	activation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_48_47498_s_14	12952965	By stimulating NHEK with cell-permeant ceramides ( e.g.D- erythro-sphingosine,  N-acetyl-(C2-ceramides)  1 or D-erythrosphingosine,  N-hexanoyl-(C6-ceramides)) it has recently been observed that ceramide-induced expression of the human ICAM-1 gene is mediated through activation of AP-2, indicating that ceramides are capable of activating transcription factors in human cells through a yet unknown mechanism ( ).	transcription
60196	7	336030	5	NULL	NULL	0	NULL	ceramide	Chemical		activates					transcription factor	GP				NULL	human cells	0	NULL	NULL	NULL	gw70_jbiolchem_278_48_47498_s_14	12952965	By stimulating NHEK with cell-permeant ceramides ( e.g.D- erythro-sphingosine,  N-acetyl-(C2-ceramides)  1 or D-erythrosphingosine,  N-hexanoyl-(C6-ceramides)) it has recently been observed that ceramide-induced expression of the human ICAM-1 gene is mediated through activation of AP-2, indicating that ceramides are capable of activating transcription factors in human cells through a yet unknown mechanism ( ).	transcription
60197	8	336030	5	NULL	NULL	0	NULL	statement 6	Process		indicates					statement 7	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_48_47498_s_14	12952965	By stimulating NHEK with cell-permeant ceramides ( e.g.D- erythro-sphingosine,  N-acetyl-(C2-ceramides)  1 or D-erythrosphingosine,  N-hexanoyl-(C6-ceramides)) it has recently been observed that ceramide-induced expression of the human ICAM-1 gene is mediated through activation of AP-2, indicating that ceramides are capable of activating transcription factors in human cells through a yet unknown mechanism ( ).	transcription
66710	1	336030	7	NULL	NULL	0	NULL	ceramide	Chemical		induce					ICAM-1 gene	GP	human;;expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_48_47498_s_14	12952965	By stimulating NHEK with cell-permeant ceramides ( e.g.D- erythro-sphingosine,  N-acetyl-(C2-ceramides)  1 or D-erythrosphingosine,  N-hexanoyl-(C6-ceramides)) it has recently been observed that ceramide-induced expression of the human ICAM-1 gene is mediated through activation of AP-2, indicating that ceramides are capable of activating transcription factors in human cells through a yet unknown mechanism ( ).	transcription
66711	2	336030	7	NULL	NULL	0	NULL	statement 1	Process		mediated through					AP-2	GP	activation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_48_47498_s_14	12952965	By stimulating NHEK with cell-permeant ceramides ( e.g.D- erythro-sphingosine,  N-acetyl-(C2-ceramides)  1 or D-erythrosphingosine,  N-hexanoyl-(C6-ceramides)) it has recently been observed that ceramide-induced expression of the human ICAM-1 gene is mediated through activation of AP-2, indicating that ceramides are capable of activating transcription factors in human cells through a yet unknown mechanism ( ).	transcription
66712	3	336030	7	NULL	NULL	0	NULL	ceramides	Chemical		activate					transcription factors	GP				NULL	human cells	0	NULL	NULL	NULL	gw70_jbiolchem_278_48_47498_s_14	12952965	By stimulating NHEK with cell-permeant ceramides ( e.g.D- erythro-sphingosine,  N-acetyl-(C2-ceramides)  1 or D-erythrosphingosine,  N-hexanoyl-(C6-ceramides)) it has recently been observed that ceramide-induced expression of the human ICAM-1 gene is mediated through activation of AP-2, indicating that ceramides are capable of activating transcription factors in human cells through a yet unknown mechanism ( ).	transcription
66713	4	336030	7	NULL	NULL	NULL	NULL	D- erythro-sphingosine	Chemical		stimulate					NHEK 	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_48_47498_s_14	12952965	By stimulating NHEK with cell-permeant ceramides ( e.g.D- erythro-sphingosine,  N-acetyl-(C2-ceramides)  1 or D-erythrosphingosine,  N-hexanoyl-(C6-ceramides)) it has recently been observed that ceramide-induced expression of the human ICAM-1 gene is mediated through activation of AP-2, indicating that ceramides are capable of activating transcription factors in human cells through a yet unknown mechanism ( ).	transcription
66714	5	336030	7	NULL	NULL	NULL	NULL	N-acetyl-(C2-ceramides)1-erythrosphingosine 	Chemical		stimulate					NHEK	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_48_47498_s_14	12952965	By stimulating NHEK with cell-permeant ceramides ( e.g.D- erythro-sphingosine,  N-acetyl-(C2-ceramides)  1 or D-erythrosphingosine,  N-hexanoyl-(C6-ceramides)) it has recently been observed that ceramide-induced expression of the human ICAM-1 gene is mediated through activation of AP-2, indicating that ceramides are capable of activating transcription factors in human cells through a yet unknown mechanism ( ).	transcription
66715	6	336030	7	NULL	NULL	NULL	NULL	N-acetyl-(C2-ceramides) D-erythrosphingosine	Chemical		stimulate					NHEK	Cell				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_48_47498_s_14	12952965	By stimulating NHEK with cell-permeant ceramides ( e.g.D- erythro-sphingosine,  N-acetyl-(C2-ceramides)  1 or D-erythrosphingosine,  N-hexanoyl-(C6-ceramides)) it has recently been observed that ceramide-induced expression of the human ICAM-1 gene is mediated through activation of AP-2, indicating that ceramides are capable of activating transcription factors in human cells through a yet unknown mechanism ( ).	transcription
66716	7	336030	7	NULL	NULL	0	NULL	N-hexanoyl-(C6-ceramides)	Chemical		stimulate					NHEK	Cell				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_48_47498_s_14	12952965	By stimulating NHEK with cell-permeant ceramides ( e.g.D- erythro-sphingosine,  N-acetyl-(C2-ceramides)  1 or D-erythrosphingosine,  N-hexanoyl-(C6-ceramides)) it has recently been observed that ceramide-induced expression of the human ICAM-1 gene is mediated through activation of AP-2, indicating that ceramides are capable of activating transcription factors in human cells through a yet unknown mechanism ( ).	transcription
66717	8	336030	7	NULL	NULL	0	NULL	D- erythro-sphingosine	Chemical		is a type of					ceramides	Chemical	cell-permeant 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_48_47498_s_14	12952965	By stimulating NHEK with cell-permeant ceramides ( e.g.D- erythro-sphingosine,  N-acetyl-(C2-ceramides)  1 or D-erythrosphingosine,  N-hexanoyl-(C6-ceramides)) it has recently been observed that ceramide-induced expression of the human ICAM-1 gene is mediated through activation of AP-2, indicating that ceramides are capable of activating transcription factors in human cells through a yet unknown mechanism ( ).	transcription
66718	9	336030	7	NULL	NULL	NULL	NULL	N-acetyl-(C2-ceramides)1-erythrosphingosine	Chemical		is a type of					ceramides	Chemical	cell-permeant 			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_48_47498_s_14	12952965	By stimulating NHEK with cell-permeant ceramides ( e.g.D- erythro-sphingosine,  N-acetyl-(C2-ceramides)  1 or D-erythrosphingosine,  N-hexanoyl-(C6-ceramides)) it has recently been observed that ceramide-induced expression of the human ICAM-1 gene is mediated through activation of AP-2, indicating that ceramides are capable of activating transcription factors in human cells through a yet unknown mechanism ( ).	transcription
66719	10	336030	7	NULL	NULL	0	NULL	N-acetyl-(C2-ceramides)D-erythrosphingosine	Chemical		is a type of					ceramides	Chemical	cell-permeant 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_48_47498_s_14	12952965	By stimulating NHEK with cell-permeant ceramides ( e.g.D- erythro-sphingosine,  N-acetyl-(C2-ceramides)  1 or D-erythrosphingosine,  N-hexanoyl-(C6-ceramides)) it has recently been observed that ceramide-induced expression of the human ICAM-1 gene is mediated through activation of AP-2, indicating that ceramides are capable of activating transcription factors in human cells through a yet unknown mechanism ( ).	transcription
66720	11	336030	7	NULL	NULL	0	NULL	N-hexanoyl-(C6-ceramides)	Chemical		is a type of					ceramide	Chemical	cell-permeant 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_48_47498_s_14	12952965	By stimulating NHEK with cell-permeant ceramides ( e.g.D- erythro-sphingosine,  N-acetyl-(C2-ceramides)  1 or D-erythrosphingosine,  N-hexanoyl-(C6-ceramides)) it has recently been observed that ceramide-induced expression of the human ICAM-1 gene is mediated through activation of AP-2, indicating that ceramides are capable of activating transcription factors in human cells through a yet unknown mechanism ( ).	transcription
60198	1	336031	5	NULL	NULL	0	NULL	hemolysis	Process		is induced by					alpha-toxin	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_196	14702348	To clarify the relationship between alpha-toxin-induced hemolysis and the deamidation of ceramide to sphingosine, the effect of  N-oleoylethanolamine ( ), a ceramidase inhibitor, on the toxin-induced hemolysis and formation of phosphorylcholine and ceramide was investigated ( Fig. 5).	transcription
60199	2	336031	5	NULL	NULL	0	NULL	ceramide	Chemical		deamidated to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_196	14702348	To clarify the relationship between alpha-toxin-induced hemolysis and the deamidation of ceramide to sphingosine, the effect of  N-oleoylethanolamine ( ), a ceramidase inhibitor, on the toxin-induced hemolysis and formation of phosphorylcholine and ceramide was investigated ( Fig. 5).	transcription
60200	3	336031	5	NULL	NULL	0	NULL	N-oleoylethanolamine	Chemical		is an inhibitor of					ceramidase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_196	14702348	To clarify the relationship between alpha-toxin-induced hemolysis and the deamidation of ceramide to sphingosine, the effect of  N-oleoylethanolamine ( ), a ceramidase inhibitor, on the toxin-induced hemolysis and formation of phosphorylcholine and ceramide was investigated ( Fig. 5).	transcription
60201	4	336031	5	NULL	NULL	0	NULL	N-oleoylethanolamine	Chemical		effects		potentially			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_196	14702348	To clarify the relationship between alpha-toxin-induced hemolysis and the deamidation of ceramide to sphingosine, the effect of  N-oleoylethanolamine ( ), a ceramidase inhibitor, on the toxin-induced hemolysis and formation of phosphorylcholine and ceramide was investigated ( Fig. 5).	transcription
60202	5	336031	5	NULL	NULL	0	NULL	N-oleoylethanolamine	Chemical		effects		potentially			phosphorylcholine	Chemical	formation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_196	14702348	To clarify the relationship between alpha-toxin-induced hemolysis and the deamidation of ceramide to sphingosine, the effect of  N-oleoylethanolamine ( ), a ceramidase inhibitor, on the toxin-induced hemolysis and formation of phosphorylcholine and ceramide was investigated ( Fig. 5).	transcription
60203	6	336031	5	NULL	NULL	0	NULL	N-oleoylethanolamine	Chemical		effects		potentially			ceramide	Chemical	formation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_196	14702348	To clarify the relationship between alpha-toxin-induced hemolysis and the deamidation of ceramide to sphingosine, the effect of  N-oleoylethanolamine ( ), a ceramidase inhibitor, on the toxin-induced hemolysis and formation of phosphorylcholine and ceramide was investigated ( Fig. 5).	transcription
66721	1	336031	7	NULL	NULL	0	NULL	alpha-toxin	GP		induce					hemolysis	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_196	14702348	To clarify the relationship between alpha-toxin-induced hemolysis and the deamidation of ceramide to sphingosine, the effect of  N-oleoylethanolamine ( ), a ceramidase inhibitor, on the toxin-induced hemolysis and formation of phosphorylcholine and ceramide was investigated ( Fig. 5).	transcription
66722	2	336031	7	NULL	NULL	0	NULL	ceramide	Chemical		deamidated to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_196	14702348	To clarify the relationship between alpha-toxin-induced hemolysis and the deamidation of ceramide to sphingosine, the effect of  N-oleoylethanolamine ( ), a ceramidase inhibitor, on the toxin-induced hemolysis and formation of phosphorylcholine and ceramide was investigated ( Fig. 5).	transcription
66723	3	336031	7	NULL	NULL	NULL	NULL	N-oleoylethanolamine	Chemical		is an inhibitor of					ceramidase 	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_13_12181_s_196	14702348	To clarify the relationship between alpha-toxin-induced hemolysis and the deamidation of ceramide to sphingosine, the effect of  N-oleoylethanolamine ( ), a ceramidase inhibitor, on the toxin-induced hemolysis and formation of phosphorylcholine and ceramide was investigated ( Fig. 5).	transcription
60204	1	336032	5	NULL	NULL	0	NULL	ceramide	Chemical		stimulates					phosphatidic acid phosphohydrolase	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_2_291_s_130	10425402	Also, ceramide stimulates the phosphatidic acid phosphohydrolase which breaks down PA as well as lyso-PA, ceramide phosphate and sphingosine thereby ablating these antagonistic signals [  62].	transcription
60205	2	336032	5	NULL	NULL	0	NULL	phosphatidic acid phosphohydrolase	GP		breaks down					PA	Chemical				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_2_291_s_130	10425402	Also, ceramide stimulates the phosphatidic acid phosphohydrolase which breaks down PA as well as lyso-PA, ceramide phosphate and sphingosine thereby ablating these antagonistic signals [  62].	transcription
60206	3	336032	5	NULL	NULL	0	NULL	phosphatidic acid phosphohydrolase	GP		breaks down					lyso-PA	Chemical				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_2_291_s_130	10425402	Also, ceramide stimulates the phosphatidic acid phosphohydrolase which breaks down PA as well as lyso-PA, ceramide phosphate and sphingosine thereby ablating these antagonistic signals [  62].	transcription
60207	4	336032	5	NULL	NULL	0	NULL	phosphatidic acid phosphohydrolase	GP		breaks down					ceramide phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_2_291_s_130	10425402	Also, ceramide stimulates the phosphatidic acid phosphohydrolase which breaks down PA as well as lyso-PA, ceramide phosphate and sphingosine thereby ablating these antagonistic signals [  62].	transcription
60208	5	336032	5	NULL	NULL	0	NULL	phosphatidic acid phosphohydrolase	GP		breaks down					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_2_291_s_130	10425402	Also, ceramide stimulates the phosphatidic acid phosphohydrolase which breaks down PA as well as lyso-PA, ceramide phosphate and sphingosine thereby ablating these antagonistic signals [  62].	transcription
66724	1	336032	7	NULL	NULL	0	NULL	 ceramide	Chemical		stimulates					phosphatidic acid phosphohydrolase	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_2_291_s_130	10425402	Also, ceramide stimulates the phosphatidic acid phosphohydrolase which breaks down PA as well as lyso-PA, ceramide phosphate and sphingosine thereby ablating these antagonistic signals [  62].	transcription
66725	2	336032	7	NULL	NULL	0	NULL	phosphatidic acid phosphohydrolase	GP		breaksdown					PA	Chemical				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_2_291_s_130	10425402	Also, ceramide stimulates the phosphatidic acid phosphohydrolase which breaks down PA as well as lyso-PA, ceramide phosphate and sphingosine thereby ablating these antagonistic signals [  62].	transcription
66726	3	336032	7	NULL	NULL	0	NULL	phosphatidic acid phosphohydrolase	GP		breaksdown					lyso-PA	Chemical				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_2_291_s_130	10425402	Also, ceramide stimulates the phosphatidic acid phosphohydrolase which breaks down PA as well as lyso-PA, ceramide phosphate and sphingosine thereby ablating these antagonistic signals [  62].	transcription
66727	4	336032	7	NULL	NULL	0	NULL	phosphatidic acid phosphohydrolase	GP		breaksdown					ceramide phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_2_291_s_130	10425402	Also, ceramide stimulates the phosphatidic acid phosphohydrolase which breaks down PA as well as lyso-PA, ceramide phosphate and sphingosine thereby ablating these antagonistic signals [  62].	transcription
66728	5	336032	7	NULL	NULL	0	NULL	phosphatidic acid phosphohydrolase	GP		breaksdown					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_2_291_s_130	10425402	Also, ceramide stimulates the phosphatidic acid phosphohydrolase which breaks down PA as well as lyso-PA, ceramide phosphate and sphingosine thereby ablating these antagonistic signals [  62].	transcription
66729	6	336032	7	NULL	NULL	0	NULL	statement 2	Process		ablate					antagonistic signals	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_2_291_s_130	10425402	Also, ceramide stimulates the phosphatidic acid phosphohydrolase which breaks down PA as well as lyso-PA, ceramide phosphate and sphingosine thereby ablating these antagonistic signals [  62].	transcription
66730	7	336032	7	NULL	NULL	0	NULL	statement 3	Process		ablate					antagonistic signals	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_2_291_s_130	10425402	Also, ceramide stimulates the phosphatidic acid phosphohydrolase which breaks down PA as well as lyso-PA, ceramide phosphate and sphingosine thereby ablating these antagonistic signals [  62].	transcription
66731	8	336032	7	NULL	NULL	0	NULL	statement 4	Process		ablate					antagonistic signals	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_2_291_s_130	10425402	Also, ceramide stimulates the phosphatidic acid phosphohydrolase which breaks down PA as well as lyso-PA, ceramide phosphate and sphingosine thereby ablating these antagonistic signals [  62].	transcription
66732	9	336032	7	NULL	NULL	0	NULL	statement 5	Process		ablate					antagonistic signals	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_2_291_s_130	10425402	Also, ceramide stimulates the phosphatidic acid phosphohydrolase which breaks down PA as well as lyso-PA, ceramide phosphate and sphingosine thereby ablating these antagonistic signals [  62].	transcription
60209	1	336033	5	NULL	NULL	0	NULL	SPP	Chemical		is converted to					sphingosine	Chemical				NULL	human fibroblasts	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_1_17_s_112	10395962	Elegantly, Gomez-Munoz et al. [ 43] demonstrated that C2-Cer stimulates the conversion of SPP to sphingosine and ceramide in human fibroblasts, whereas Rani et al. [ 29] showed that C2-Cer is able to increase the endogenous ceramide content.	transcription
60210	2	336033	5	NULL	NULL	0	NULL	SPP	Chemical		is converted to					ceramide	Chemical				NULL	human fibroblasts	0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_1_17_s_112	10395962	Elegantly, Gomez-Munoz et al. [ 43] demonstrated that C2-Cer stimulates the conversion of SPP to sphingosine and ceramide in human fibroblasts, whereas Rani et al. [ 29] showed that C2-Cer is able to increase the endogenous ceramide content.	transcription
60211	3	336033	5	NULL	NULL	0	NULL	C2-Cer	Chemical		stimulates					statement 1	Process				NULL	human fibroblasts	0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_1_17_s_112	10395962	Elegantly, Gomez-Munoz et al. [ 43] demonstrated that C2-Cer stimulates the conversion of SPP to sphingosine and ceramide in human fibroblasts, whereas Rani et al. [ 29] showed that C2-Cer is able to increase the endogenous ceramide content.	transcription
60212	4	336033	5	NULL	NULL	0	NULL	C2-Cer	Chemical		stimulates					statement 2	Process				NULL	human fibroblasts	0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_1_17_s_112	10395962	Elegantly, Gomez-Munoz et al. [ 43] demonstrated that C2-Cer stimulates the conversion of SPP to sphingosine and ceramide in human fibroblasts, whereas Rani et al. [ 29] showed that C2-Cer is able to increase the endogenous ceramide content.	transcription
60213	5	336033	5	NULL	NULL	0	NULL	C2-Cer	Chemical		increases					ceramide	Chemical	endogenous			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_1_17_s_112	10395962	Elegantly, Gomez-Munoz et al. [ 43] demonstrated that C2-Cer stimulates the conversion of SPP to sphingosine and ceramide in human fibroblasts, whereas Rani et al. [ 29] showed that C2-Cer is able to increase the endogenous ceramide content.	transcription
66733	1	336033	7	NULL	NULL	NULL	NULL	 SPP	Chemical		converted to					sphingosine	Chemical				NULL	human fibroblasts	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_1_17_s_112	10395962	Elegantly, Gomez-Munoz et al. [ 43] demonstrated that C2-Cer stimulates the conversion of SPP to sphingosine and ceramide in human fibroblasts, whereas Rani et al. [ 29] showed that C2-Cer is able to increase the endogenous ceramide content.	transcription
66734	2	336033	7	NULL	NULL	0	NULL	 SPP	Chemical		converted to					ceramide	Chemical				NULL	human fibroblasts	0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_1_17_s_112	10395962	Elegantly, Gomez-Munoz et al. [ 43] demonstrated that C2-Cer stimulates the conversion of SPP to sphingosine and ceramide in human fibroblasts, whereas Rani et al. [ 29] showed that C2-Cer is able to increase the endogenous ceramide content.	transcription
66735	3	336033	7	NULL	NULL	NULL	NULL	C2-Cer	Chemical		stimulate					statement 1	Process				NULL	human fibroblasts	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_1_17_s_112	10395962	Elegantly, Gomez-Munoz et al. [ 43] demonstrated that C2-Cer stimulates the conversion of SPP to sphingosine and ceramide in human fibroblasts, whereas Rani et al. [ 29] showed that C2-Cer is able to increase the endogenous ceramide content.	transcription
66736	4	336033	7	NULL	NULL	NULL	NULL	C2-Cer	Chemical		stimulate					statement 2	Chemical				NULL	human fibroblasts	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_1_17_s_112	10395962	Elegantly, Gomez-Munoz et al. [ 43] demonstrated that C2-Cer stimulates the conversion of SPP to sphingosine and ceramide in human fibroblasts, whereas Rani et al. [ 29] showed that C2-Cer is able to increase the endogenous ceramide content.	transcription
66737	5	336033	7	NULL	NULL	0	NULL	C2-Cer	Chemical		increase					ceramide content	Process	endogenous			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_1_17_s_112	10395962	Elegantly, Gomez-Munoz et al. [ 43] demonstrated that C2-Cer stimulates the conversion of SPP to sphingosine and ceramide in human fibroblasts, whereas Rani et al. [ 29] showed that C2-Cer is able to increase the endogenous ceramide content.	transcription
66738	6	336033	7	NULL	NULL	0	NULL	C2-Cer	Chemical		increase					ceramide content	Process	endogenous			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1439_1_17_s_112	10395962	Elegantly, Gomez-Munoz et al. [ 43] demonstrated that C2-Cer stimulates the conversion of SPP to sphingosine and ceramide in human fibroblasts, whereas Rani et al. [ 29] showed that C2-Cer is able to increase the endogenous ceramide content.	transcription
60214	1	336034	5	NULL	NULL	0	NULL	ceramide	Chemical		is induced by					daunorubicin	Chemical				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1488_3_219_s_221	11082532	To exclude the possibility that daunorubicin-induced ceramide was rapidly hydrolyzed to sphingosine by ceramidase and therefore its increase could not be detected, we measured the ceramide generation in A-431 cells treated with daunorubicin in the presence of  N-oleoylethanolamine, a ceramidase inhibitor.	transcription
60215	2	336034	5	NULL	NULL	0	NULL	statement 1	Chemical		is hydrolyzed to		rapidly			sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1488_3_219_s_221	11082532	To exclude the possibility that daunorubicin-induced ceramide was rapidly hydrolyzed to sphingosine by ceramidase and therefore its increase could not be detected, we measured the ceramide generation in A-431 cells treated with daunorubicin in the presence of  N-oleoylethanolamine, a ceramidase inhibitor.	transcription
60216	3	336034	5	NULL	NULL	0	NULL	ceramidase	GP		catalyzes					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1488_3_219_s_221	11082532	To exclude the possibility that daunorubicin-induced ceramide was rapidly hydrolyzed to sphingosine by ceramidase and therefore its increase could not be detected, we measured the ceramide generation in A-431 cells treated with daunorubicin in the presence of  N-oleoylethanolamine, a ceramidase inhibitor.	transcription
60217	4	336034	5	NULL	NULL	0	NULL	N-oleoylethanolamine	Chemical		is an inhibitor of					ceramidase	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1488_3_219_s_221	11082532	To exclude the possibility that daunorubicin-induced ceramide was rapidly hydrolyzed to sphingosine by ceramidase and therefore its increase could not be detected, we measured the ceramide generation in A-431 cells treated with daunorubicin in the presence of  N-oleoylethanolamine, a ceramidase inhibitor.	transcription
66746	1	336034	7	NULL	NULL	0	NULL	daunorubicin	Chemical		induce					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1488_3_219_s_221	11082532	To exclude the possibility that daunorubicin-induced ceramide was rapidly hydrolyzed to sphingosine by ceramidase and therefore its increase could not be detected, we measured the ceramide generation in A-431 cells treated with daunorubicin in the presence of  N-oleoylethanolamine, a ceramidase inhibitor.	transcription
66747	2	336034	7	NULL	NULL	0	NULL	statement 1	Process		hydrolyze to		rapidly			sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1488_3_219_s_221	11082532	To exclude the possibility that daunorubicin-induced ceramide was rapidly hydrolyzed to sphingosine by ceramidase and therefore its increase could not be detected, we measured the ceramide generation in A-431 cells treated with daunorubicin in the presence of  N-oleoylethanolamine, a ceramidase inhibitor.	transcription
66748	3	336034	7	NULL	NULL	0	NULL	ceramidase	GP		catalyze					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1488_3_219_s_221	11082532	To exclude the possibility that daunorubicin-induced ceramide was rapidly hydrolyzed to sphingosine by ceramidase and therefore its increase could not be detected, we measured the ceramide generation in A-431 cells treated with daunorubicin in the presence of  N-oleoylethanolamine, a ceramidase inhibitor.	transcription
66749	4	336034	7	NULL	NULL	0	NULL	N-oleoylethanolamine	Chemical		is an inhibitor of					ceramidase	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1488_3_219_s_221	11082532	To exclude the possibility that daunorubicin-induced ceramide was rapidly hydrolyzed to sphingosine by ceramidase and therefore its increase could not be detected, we measured the ceramide generation in A-431 cells treated with daunorubicin in the presence of  N-oleoylethanolamine, a ceramidase inhibitor.	transcription
60218	1	336035	5	NULL	NULL	0	NULL	FB1	Chemical		is an inhibitor of					ceramide synthase	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_158_6_1039_s_187	12235122	Yet, FB1, an inhibitor of ceramide synthase, induced accumulation of sphingoid bases when cells were treated with either S1P or dihydro-S1P, suggesting that the sphingosine and sphinganine produced in these cells are indeed substrates for ceramide synthase.	transcription
60219	2	336035	5	NULL	NULL	0	NULL	FB1	Chemical		induce					sphingoid bases	Chemical	accumulation of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_158_6_1039_s_187	12235122	Yet, FB1, an inhibitor of ceramide synthase, induced accumulation of sphingoid bases when cells were treated with either S1P or dihydro-S1P, suggesting that the sphingosine and sphinganine produced in these cells are indeed substrates for ceramide synthase.	transcription
60220	3	336035	5	NULL	NULL	0	NULL	statement 2	Process		occurs upon					S1P	Chemical	treatment			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_158_6_1039_s_187	12235122	Yet, FB1, an inhibitor of ceramide synthase, induced accumulation of sphingoid bases when cells were treated with either S1P or dihydro-S1P, suggesting that the sphingosine and sphinganine produced in these cells are indeed substrates for ceramide synthase.	transcription
60221	4	336035	5	NULL	NULL	0	NULL	statement 2	Process		occurs upon					dihydro-S1P	Chemical	treatment			NULL		0	NULL	NULL	NULL	gw60_cellbiol_158_6_1039_s_187	12235122	Yet, FB1, an inhibitor of ceramide synthase, induced accumulation of sphingoid bases when cells were treated with either S1P or dihydro-S1P, suggesting that the sphingosine and sphinganine produced in these cells are indeed substrates for ceramide synthase.	transcription
60222	5	336035	5	NULL	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_158_6_1039_s_187	12235122	Yet, FB1, an inhibitor of ceramide synthase, induced accumulation of sphingoid bases when cells were treated with either S1P or dihydro-S1P, suggesting that the sphingosine and sphinganine produced in these cells are indeed substrates for ceramide synthase.	transcription
60223	6	336035	5	NULL	NULL	0	NULL	sphingosine	Chemical		is a substrate of					ceramide synthase	GP				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_158_6_1039_s_187	12235122	Yet, FB1, an inhibitor of ceramide synthase, induced accumulation of sphingoid bases when cells were treated with either S1P or dihydro-S1P, suggesting that the sphingosine and sphinganine produced in these cells are indeed substrates for ceramide synthase.	transcription
60224	7	336035	5	NULL	NULL	0	NULL	sphinganine	Chemical		is a substrate of					ceramide synthase	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_158_6_1039_s_187	12235122	Yet, FB1, an inhibitor of ceramide synthase, induced accumulation of sphingoid bases when cells were treated with either S1P or dihydro-S1P, suggesting that the sphingosine and sphinganine produced in these cells are indeed substrates for ceramide synthase.	transcription
66750	1	336035	7	NULL	NULL	0	NULL	FB1	Chemical		is an inhibitor of					ceramide synthase	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_158_6_1039_s_187	12235122	Yet, FB1, an inhibitor of ceramide synthase, induced accumulation of sphingoid bases when cells were treated with either S1P or dihydro-S1P, suggesting that the sphingosine and sphinganine produced in these cells are indeed substrates for ceramide synthase.	transcription
66751	2	336035	7	NULL	NULL	0	NULL	FB1	Chemical		induce					sphingoid bases	Chemical	accumulation of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_158_6_1039_s_187	12235122	Yet, FB1, an inhibitor of ceramide synthase, induced accumulation of sphingoid bases when cells were treated with either S1P or dihydro-S1P, suggesting that the sphingosine and sphinganine produced in these cells are indeed substrates for ceramide synthase.	transcription
66752	3	336035	7	NULL	NULL	0	NULL	statement 2	Process		occur upon					S1P	Chemical	treatment with			NULL		0	NULL	NULL	NULL	gw60_cellbiol_158_6_1039_s_187	12235122	Yet, FB1, an inhibitor of ceramide synthase, induced accumulation of sphingoid bases when cells were treated with either S1P or dihydro-S1P, suggesting that the sphingosine and sphinganine produced in these cells are indeed substrates for ceramide synthase.	transcription
66753	4	336035	7	NULL	NULL	NULL	NULL	statement 2	Process		occur upon					dihydro-S1P	Chemical	treatment with			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_158_6_1039_s_187	12235122	Yet, FB1, an inhibitor of ceramide synthase, induced accumulation of sphingoid bases when cells were treated with either S1P or dihydro-S1P, suggesting that the sphingosine and sphinganine produced in these cells are indeed substrates for ceramide synthase.	transcription
66754	5	336035	7	NULL	NULL	0	NULL	sphingosine	Chemical		substrate for					ceramide synthase	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_158_6_1039_s_187	12235122	Yet, FB1, an inhibitor of ceramide synthase, induced accumulation of sphingoid bases when cells were treated with either S1P or dihydro-S1P, suggesting that the sphingosine and sphinganine produced in these cells are indeed substrates for ceramide synthase.	transcription
66755	6	336035	7	NULL	NULL	0	NULL	sphinganine 	Chemical		substrate for					ceramide synthase	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_158_6_1039_s_187	12235122	Yet, FB1, an inhibitor of ceramide synthase, induced accumulation of sphingoid bases when cells were treated with either S1P or dihydro-S1P, suggesting that the sphingosine and sphinganine produced in these cells are indeed substrates for ceramide synthase.	transcription
60225	1	336036	5	NULL	NULL	0	NULL	1 ,25(OH)2D3	Chemical		activates					sphingosine kinase	GP				NULL		0	NULL	NULL	NULL	gw60_chembiol_7_3_173_s_236	10712934	It has been shown that 1 ,25(OH)2D3 activates sphingosine kinase, which in turn converts ceramide to sphingosin-1-phosphate (SPP) and prevents HL-60 cell ceramide-induced apoptosis  [50]  .	transcription
60226	2	336036	5	NULL	NULL	0	NULL	ceramide	Chemical		is converted to					SPP	Chemical				NULL		0	NULL	NULL	NULL	gw60_chembiol_7_3_173_s_236	10712934	It has been shown that 1 ,25(OH)2D3 activates sphingosine kinase, which in turn converts ceramide to sphingosin-1-phosphate (SPP) and prevents HL-60 cell ceramide-induced apoptosis  [50]  .	transcription
60227	3	336036	5	NULL	NULL	0	NULL	SPP	Chemical		is					sphingosin-1-phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_chembiol_7_3_173_s_236	10712934	It has been shown that 1 ,25(OH)2D3 activates sphingosine kinase, which in turn converts ceramide to sphingosin-1-phosphate (SPP) and prevents HL-60 cell ceramide-induced apoptosis  [50]  .	transcription
60228	4	336036	5	NULL	NULL	0	NULL	sphingosine kinase	GP	activated	catalyzes					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_chembiol_7_3_173_s_236	10712934	It has been shown that 1 ,25(OH)2D3 activates sphingosine kinase, which in turn converts ceramide to sphingosin-1-phosphate (SPP) and prevents HL-60 cell ceramide-induced apoptosis  [50]  .	transcription
60229	5	336036	5	NULL	NULL	0	NULL	apoptosis	Process		is induced by					ceramide	Chemical				NULL	HL-60 cell	0	NULL	NULL	NULL	gw60_chembiol_7_3_173_s_236	10712934	It has been shown that 1 ,25(OH)2D3 activates sphingosine kinase, which in turn converts ceramide to sphingosin-1-phosphate (SPP) and prevents HL-60 cell ceramide-induced apoptosis  [50]  .	transcription
60230	6	336036	5	NULL	NULL	0	NULL	statement 2	Process		prevents					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_chembiol_7_3_173_s_236	10712934	It has been shown that 1 ,25(OH)2D3 activates sphingosine kinase, which in turn converts ceramide to sphingosin-1-phosphate (SPP) and prevents HL-60 cell ceramide-induced apoptosis  [50]  .	transcription
66850	1	336036	7	NULL	NULL	0	NULL	1 ,25(OH)2D3	Chemical		activates					sphingosine kinase	GP				NULL		0	NULL	NULL	NULL	gw60_chembiol_7_3_173_s_236	10712934	It has been shown that 1 ,25(OH)2D3 activates sphingosine kinase, which in turn converts ceramide to sphingosin-1-phosphate (SPP) and prevents HL-60 cell ceramide-induced apoptosis  [50]  .	transcription
66851	2	336036	7	NULL	NULL	0	NULL	ceramide	Chemical		converted to					SPP	Chemical				NULL		0	NULL	NULL	NULL	gw60_chembiol_7_3_173_s_236	10712934	It has been shown that 1 ,25(OH)2D3 activates sphingosine kinase, which in turn converts ceramide to sphingosin-1-phosphate (SPP) and prevents HL-60 cell ceramide-induced apoptosis  [50]  .	transcription
66852	3	336036	7	NULL	NULL	NULL	NULL	sphingosine kinase	GP		catalyze					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_7_3_173_s_236	10712934	It has been shown that 1 ,25(OH)2D3 activates sphingosine kinase, which in turn converts ceramide to sphingosin-1-phosphate (SPP) and prevents HL-60 cell ceramide-induced apoptosis  [50]  .	transcription
66853	4	336036	7	NULL	NULL	NULL	NULL	ceramide	Chemical	HL-60 cell 	induce					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_chembiol_7_3_173_s_236	10712934	It has been shown that 1 ,25(OH)2D3 activates sphingosine kinase, which in turn converts ceramide to sphingosin-1-phosphate (SPP) and prevents HL-60 cell ceramide-induced apoptosis  [50]  .	transcription
66854	5	336036	7	NULL	NULL	0	NULL	sphingosine kinase	GP		prevents					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_chembiol_7_3_173_s_236	10712934	It has been shown that 1 ,25(OH)2D3 activates sphingosine kinase, which in turn converts ceramide to sphingosin-1-phosphate (SPP) and prevents HL-60 cell ceramide-induced apoptosis  [50]  .	transcription
66855	6	336036	7	NULL	NULL	0	NULL	SPP	Chemical		is					sphingosin-1-phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_chembiol_7_3_173_s_236	10712934	It has been shown that 1 ,25(OH)2D3 activates sphingosine kinase, which in turn converts ceramide to sphingosin-1-phosphate (SPP) and prevents HL-60 cell ceramide-induced apoptosis  [50]  .	transcription
60231	1	336037	5	NULL	NULL	0	NULL	ceramide	Chemical	levels of	is induced by					LPS	Chemical				NULL	mice	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_34_30784_s_242	12072440	First we showed that old MO have significantly higher LPS-induced ceramide levels compared with young mice, whereas there is no age difference in ceramide downstream metabolite sphingosine.	transcription
60232	2	336037	5	NULL	NULL	0	NULL	sphingosine	Chemical		is a metabolite of					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_34_30784_s_242	12072440	First we showed that old MO have significantly higher LPS-induced ceramide levels compared with young mice, whereas there is no age difference in ceramide downstream metabolite sphingosine.	transcription
66856	1	336037	7	NULL	NULL	0	NULL	 LPS	Chemical		induce					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_34_30784_s_242	12072440	First we showed that old MO have significantly higher LPS-induced ceramide levels compared with young mice, whereas there is no age difference in ceramide downstream metabolite sphingosine.	transcription
66857	2	336037	7	NULL	NULL	NULL	NULL	sphingosine	Chemical		is downstream metabolite of					ceramide	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_34_30784_s_242	12072440	First we showed that old MO have significantly higher LPS-induced ceramide levels compared with young mice, whereas there is no age difference in ceramide downstream metabolite sphingosine.	transcription
60245	1	336038	5	NULL	NULL	0	NULL	neurons	Cell	 death of	is induced by					NGF	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_12_9812_s_149	11777929	Ceramide Itself, and Not a Downstream Lipid Metabolite, Signals NGF-induced Neuronal Death-- Ceramide can be degraded by ceramidases to downstream metabolites such as sphingosine 1-phosphate, which has been shown to act as an extracellular initiator of apoptosis ( 47,  48).	transcription
60246	2	336038	5	NULL	NULL	0	NULL	ceramide	Chemical		signals					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_12_9812_s_149	11777929	Ceramide Itself, and Not a Downstream Lipid Metabolite, Signals NGF-induced Neuronal Death-- Ceramide can be degraded by ceramidases to downstream metabolites such as sphingosine 1-phosphate, which has been shown to act as an extracellular initiator of apoptosis ( 47,  48).	transcription
60247	3	336038	5	NULL	NULL	0	NULL	ceramide	Chemical		is degraded to					sphingosine 1-phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_12_9812_s_149	11777929	Ceramide Itself, and Not a Downstream Lipid Metabolite, Signals NGF-induced Neuronal Death-- Ceramide can be degraded by ceramidases to downstream metabolites such as sphingosine 1-phosphate, which has been shown to act as an extracellular initiator of apoptosis ( 47,  48).	transcription
60248	4	336038	5	NULL	NULL	0	NULL	ceramidases	GP		catalyzes					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_12_9812_s_149	11777929	Ceramide Itself, and Not a Downstream Lipid Metabolite, Signals NGF-induced Neuronal Death-- Ceramide can be degraded by ceramidases to downstream metabolites such as sphingosine 1-phosphate, which has been shown to act as an extracellular initiator of apoptosis ( 47,  48).	transcription
60249	5	336038	5	NULL	NULL	0	NULL	sphingosine 1-phosphate	Chemical		is an initiator of					apoptosis	Process				NULL	extracellularly	0	NULL	NULL	NULL	gw60_jbiolchem_277_12_9812_s_149	11777929	Ceramide Itself, and Not a Downstream Lipid Metabolite, Signals NGF-induced Neuronal Death-- Ceramide can be degraded by ceramidases to downstream metabolites such as sphingosine 1-phosphate, which has been shown to act as an extracellular initiator of apoptosis ( 47,  48).	transcription
66858	1	336038	7	NULL	NULL	0	NULL	NGF	GP		induce					Neuronal death	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_12_9812_s_149	11777929	Ceramide Itself, and Not a Downstream Lipid Metabolite, Signals NGF-induced Neuronal Death-- Ceramide can be degraded by ceramidases to downstream metabolites such as sphingosine 1-phosphate, which has been shown to act as an extracellular initiator of apoptosis ( 47,  48).	transcription
66859	2	336038	7	NULL	NULL	0	NULL	ceramide	Chemical		degraded to					sphingosine 1-phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_12_9812_s_149	11777929	Ceramide Itself, and Not a Downstream Lipid Metabolite, Signals NGF-induced Neuronal Death-- Ceramide can be degraded by ceramidases to downstream metabolites such as sphingosine 1-phosphate, which has been shown to act as an extracellular initiator of apoptosis ( 47,  48).	transcription
66860	3	336038	7	NULL	NULL	0	NULL	ceramidases	GP		catalyze					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_12_9812_s_149	11777929	Ceramide Itself, and Not a Downstream Lipid Metabolite, Signals NGF-induced Neuronal Death-- Ceramide can be degraded by ceramidases to downstream metabolites such as sphingosine 1-phosphate, which has been shown to act as an extracellular initiator of apoptosis ( 47,  48).	transcription
66861	4	336038	7	NULL	NULL	0	NULL	sphingosine 1-phosphate	Chemical		act as an					apoptosis	Process	extracellular initiator of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_12_9812_s_149	11777929	Ceramide Itself, and Not a Downstream Lipid Metabolite, Signals NGF-induced Neuronal Death-- Ceramide can be degraded by ceramidases to downstream metabolites such as sphingosine 1-phosphate, which has been shown to act as an extracellular initiator of apoptosis ( 47,  48).	transcription
60259	1	336039	5	NULL	NULL	0	NULL	ceramide	Chemical		is hydrolyzed to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23294_s_23	11956206	Although termination of the second messenger actions of ceramide is considered to be mediated by ceramidase, which hydrolyzes it to form sphingosine, it was suggested more than a decade ago that ceramide can also be phosphorylated to ceramide-1-phosphate ( 22).	transcription
60260	2	336039	5	NULL	NULL	0	NULL	ceramidase	GP		catalyzes					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23294_s_23	11956206	Although termination of the second messenger actions of ceramide is considered to be mediated by ceramidase, which hydrolyzes it to form sphingosine, it was suggested more than a decade ago that ceramide can also be phosphorylated to ceramide-1-phosphate ( 22).	transcription
60261	3	336039	5	NULL	NULL	0	NULL	ceramide	Chemical		is phosphorylated to					ceramide-1-phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23294_s_23	11956206	Although termination of the second messenger actions of ceramide is considered to be mediated by ceramidase, which hydrolyzes it to form sphingosine, it was suggested more than a decade ago that ceramide can also be phosphorylated to ceramide-1-phosphate ( 22).	transcription
66866	1	336039	7	NULL	NULL	0	NULL	ceramide	Chemical		hydrolyzed to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23294_s_23	11956206	Although termination of the second messenger actions of ceramide is considered to be mediated by ceramidase, which hydrolyzes it to form sphingosine, it was suggested more than a decade ago that ceramide can also be phosphorylated to ceramide-1-phosphate ( 22).	transcription
66867	2	336039	7	NULL	NULL	0	NULL	ceramidase	GP		catalyze					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23294_s_23	11956206	Although termination of the second messenger actions of ceramide is considered to be mediated by ceramidase, which hydrolyzes it to form sphingosine, it was suggested more than a decade ago that ceramide can also be phosphorylated to ceramide-1-phosphate ( 22).	transcription
66868	3	336039	7	NULL	NULL	0	NULL	ceramidase	GP		mediates					second messenger actions	Process	termination of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23294_s_23	11956206	Although termination of the second messenger actions of ceramide is considered to be mediated by ceramidase, which hydrolyzes it to form sphingosine, it was suggested more than a decade ago that ceramide can also be phosphorylated to ceramide-1-phosphate ( 22).	transcription
66869	4	336039	7	NULL	NULL	NULL	NULL	statement 3	Process		occur through					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_26_23294_s_23	11956206	Although termination of the second messenger actions of ceramide is considered to be mediated by ceramidase, which hydrolyzes it to form sphingosine, it was suggested more than a decade ago that ceramide can also be phosphorylated to ceramide-1-phosphate ( 22).	transcription
66871	5	336039	7	NULL	NULL	0	NULL	ceramide	Chemical		phosphorylated to					ceramide-1-phosphate 	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23294_s_23	11956206	Although termination of the second messenger actions of ceramide is considered to be mediated by ceramidase, which hydrolyzes it to form sphingosine, it was suggested more than a decade ago that ceramide can also be phosphorylated to ceramide-1-phosphate ( 22).	transcription
60262	1	336040	5	NULL	NULL	0	NULL	S1P	Chemical		is implicated in					cell growth	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_36_32947_s_21	12080051	In contrast to the growth inhibitory and pro-apoptotic effects of ceramide and sphingosine, a further metabolite, S1P, has been implicated in cell growth ( 7) and inhibition of ceramide-mediated apoptosis ( 8-13).	transcription
60264	2	336040	5	NULL	NULL	0	NULL	apoptosis	Process		is mediated by					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_36_32947_s_21	12080051	In contrast to the growth inhibitory and pro-apoptotic effects of ceramide and sphingosine, a further metabolite, S1P, has been implicated in cell growth ( 7) and inhibition of ceramide-mediated apoptosis ( 8-13).	transcription
60265	3	336040	5	NULL	NULL	0	NULL	S1P	Chemical		inhibits					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_36_32947_s_21	12080051	In contrast to the growth inhibitory and pro-apoptotic effects of ceramide and sphingosine, a further metabolite, S1P, has been implicated in cell growth ( 7) and inhibition of ceramide-mediated apoptosis ( 8-13).	transcription
66874	1	336040	7	NULL	NULL	0	NULL	ceramide	Chemical		inhibits					growth	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_36_32947_s_21	12080051	In contrast to the growth inhibitory and pro-apoptotic effects of ceramide and sphingosine, a further metabolite, S1P, has been implicated in cell growth ( 7) and inhibition of ceramide-mediated apoptosis ( 8-13).	transcription
66882	2	336040	7	NULL	NULL	0	NULL	ceramide	Chemical		effect					pro-apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_36_32947_s_21	12080051	In contrast to the growth inhibitory and pro-apoptotic effects of ceramide and sphingosine, a further metabolite, S1P, has been implicated in cell growth ( 7) and inhibition of ceramide-mediated apoptosis ( 8-13).	transcription
66885	3	336040	7	NULL	NULL	0	NULL	sphingosine	Chemical		inhibits					growth	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_36_32947_s_21	12080051	In contrast to the growth inhibitory and pro-apoptotic effects of ceramide and sphingosine, a further metabolite, S1P, has been implicated in cell growth ( 7) and inhibition of ceramide-mediated apoptosis ( 8-13).	transcription
66886	4	336040	7	NULL	NULL	0	NULL	sphingosine	Chemical		effect					pro-apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_36_32947_s_21	12080051	In contrast to the growth inhibitory and pro-apoptotic effects of ceramide and sphingosine, a further metabolite, S1P, has been implicated in cell growth ( 7) and inhibition of ceramide-mediated apoptosis ( 8-13).	transcription
66887	5	336040	7	NULL	NULL	0	NULL	S1P	Chemical		implicated in					cell growth	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_36_32947_s_21	12080051	In contrast to the growth inhibitory and pro-apoptotic effects of ceramide and sphingosine, a further metabolite, S1P, has been implicated in cell growth ( 7) and inhibition of ceramide-mediated apoptosis ( 8-13).	transcription
66888	6	336040	7	NULL	NULL	0	NULL	ceramide	Chemical		mediate					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_36_32947_s_21	12080051	In contrast to the growth inhibitory and pro-apoptotic effects of ceramide and sphingosine, a further metabolite, S1P, has been implicated in cell growth ( 7) and inhibition of ceramide-mediated apoptosis ( 8-13).	transcription
66896	7	336040	7	NULL	NULL	0	NULL	S1P	Chemical		inhibit					statement 6					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_36_32947_s_21	12080051	In contrast to the growth inhibitory and pro-apoptotic effects of ceramide and sphingosine, a further metabolite, S1P, has been implicated in cell growth ( 7) and inhibition of ceramide-mediated apoptosis ( 8-13).	transcription
60266	1	336041	5	NULL	NULL	0	NULL	ceramidases	GP		regulates					ceramide	Chemical	level of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_25847_s_108	12011103	For example, ceramidases can regulate the levels of ceramide (substrate) and/or sphingosine and S1P (products), with S1P often exerting anti-apoptotic effects that antagonize ceramide-mediated responses (see minireview by Spiegel and Milstien ( 58)).	transcription
60267	2	336041	5	NULL	NULL	0	NULL	ceramidases	GP		regulates					sphingosine	Chemical	level of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_25847_s_108	12011103	For example, ceramidases can regulate the levels of ceramide (substrate) and/or sphingosine and S1P (products), with S1P often exerting anti-apoptotic effects that antagonize ceramide-mediated responses (see minireview by Spiegel and Milstien ( 58)).	transcription
60268	3	336041	5	NULL	NULL	0	NULL	ceramidases	GP		regulates					S1P	Chemical	level of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_25847_s_108	12011103	For example, ceramidases can regulate the levels of ceramide (substrate) and/or sphingosine and S1P (products), with S1P often exerting anti-apoptotic effects that antagonize ceramide-mediated responses (see minireview by Spiegel and Milstien ( 58)).	transcription
66897	1	336041	7	NULL	NULL	0	NULL	ceramidases	GP		regulate					ceramide	Chemical	levels of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_25847_s_108	12011103	For example, ceramidases can regulate the levels of ceramide (substrate) and/or sphingosine and S1P (products), with S1P often exerting anti-apoptotic effects that antagonize ceramide-mediated responses (see minireview by Spiegel and Milstien ( 58)).	transcription
66898	2	336041	7	NULL	NULL	0	NULL	ceramidases	GP		regulate					sphingosine	Chemical	levels of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_25847_s_108	12011103	For example, ceramidases can regulate the levels of ceramide (substrate) and/or sphingosine and S1P (products), with S1P often exerting anti-apoptotic effects that antagonize ceramide-mediated responses (see minireview by Spiegel and Milstien ( 58)).	transcription
66899	3	336041	7	NULL	NULL	0	NULL	ceramidases	GP		regulate					S1P	Chemical	levels of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_25847_s_108	12011103	For example, ceramidases can regulate the levels of ceramide (substrate) and/or sphingosine and S1P (products), with S1P often exerting anti-apoptotic effects that antagonize ceramide-mediated responses (see minireview by Spiegel and Milstien ( 58)).	transcription
66900	4	336041	7	NULL	NULL	0	NULL	S1P	Chemical		exerts					anti-apoptotic effects	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_25847_s_108	12011103	For example, ceramidases can regulate the levels of ceramide (substrate) and/or sphingosine and S1P (products), with S1P often exerting anti-apoptotic effects that antagonize ceramide-mediated responses (see minireview by Spiegel and Milstien ( 58)).	transcription
66901	5	336041	7	NULL	NULL	0	NULL	ceramide	Chemical		mediate					responses	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_25847_s_108	12011103	For example, ceramidases can regulate the levels of ceramide (substrate) and/or sphingosine and S1P (products), with S1P often exerting anti-apoptotic effects that antagonize ceramide-mediated responses (see minireview by Spiegel and Milstien ( 58)).	transcription
66902	6	336041	7	NULL	NULL	0	NULL	S1P	Chemical		antagonize					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_29_25847_s_108	12011103	For example, ceramidases can regulate the levels of ceramide (substrate) and/or sphingosine and S1P (products), with S1P often exerting anti-apoptotic effects that antagonize ceramide-mediated responses (see minireview by Spiegel and Milstien ( 58)).	transcription
60275	1	336042	5	NULL	NULL	0	NULL	PLA2	GP		does not induce		significantly			JNK	GP	activity of			NULL	MS1418 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_44_27753_s_70	9346918	In contrast, PLA2 or PLC did not show significant induction of JNK activity, and C2-Dhc (an inactive form of ceramide) or sphingosine (a metabolic of ceramide) induces only very weak JNK activation in MS1418 cells (Fig.  6).	transcription
60276	2	336042	5	NULL	NULL	0	NULL	PLC	GP		does not induce		significantly			JNK	GP	activity of			NULL	MS1418 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_44_27753_s_70	9346918	In contrast, PLA2 or PLC did not show significant induction of JNK activity, and C2-Dhc (an inactive form of ceramide) or sphingosine (a metabolic of ceramide) induces only very weak JNK activation in MS1418 cells (Fig.  6).	transcription
60277	3	336042	5	NULL	NULL	0	NULL	C2-Dhc	Chemical		is an inactive form of					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27753_s_70	9346918	In contrast, PLA2 or PLC did not show significant induction of JNK activity, and C2-Dhc (an inactive form of ceramide) or sphingosine (a metabolic of ceramide) induces only very weak JNK activation in MS1418 cells (Fig.  6).	transcription
60278	4	336042	5	NULL	NULL	0	NULL	C2-Dhc	Chemical		induce		weakly			JNK	GP	activation of			NULL	MS1418 cells	0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27753_s_70	9346918	In contrast, PLA2 or PLC did not show significant induction of JNK activity, and C2-Dhc (an inactive form of ceramide) or sphingosine (a metabolic of ceramide) induces only very weak JNK activation in MS1418 cells (Fig.  6).	transcription
60279	5	336042	5	NULL	NULL	0	NULL	sphingosine	Chemical		induce		weakly			JNK	GP	activation of			NULL	MS1418 cells	0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27753_s_70	9346918	In contrast, PLA2 or PLC did not show significant induction of JNK activity, and C2-Dhc (an inactive form of ceramide) or sphingosine (a metabolic of ceramide) induces only very weak JNK activation in MS1418 cells (Fig.  6).	transcription
60281	6	336042	5	NULL	NULL	0	NULL	sphingosine	Chemical		is a metabolite of					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27753_s_70	9346918	In contrast, PLA2 or PLC did not show significant induction of JNK activity, and C2-Dhc (an inactive form of ceramide) or sphingosine (a metabolic of ceramide) induces only very weak JNK activation in MS1418 cells (Fig.  6).	transcription
66903	1	336042	7	NULL	NULL	0	NULL	PLA2	Chemical		does not induce		significantly			JNK activity	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27753_s_70	9346918	In contrast, PLA2 or PLC did not show significant induction of JNK activity, and C2-Dhc (an inactive form of ceramide) or sphingosine (a metabolic of ceramide) induces only very weak JNK activation in MS1418 cells (Fig.  6).	transcription
66904	2	336042	7	NULL	NULL	0	NULL	PLC 	Chemical		does not induce		significantly			JNK activity	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27753_s_70	9346918	In contrast, PLA2 or PLC did not show significant induction of JNK activity, and C2-Dhc (an inactive form of ceramide) or sphingosine (a metabolic of ceramide) induces only very weak JNK activation in MS1418 cells (Fig.  6).	transcription
66905	3	336042	7	NULL	NULL	0	NULL	C2-Dhc	Chemical		is inactive form of					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27753_s_70	9346918	In contrast, PLA2 or PLC did not show significant induction of JNK activity, and C2-Dhc (an inactive form of ceramide) or sphingosine (a metabolic of ceramide) induces only very weak JNK activation in MS1418 cells (Fig.  6).	transcription
66906	4	336042	7	NULL	NULL	0	NULL	C2-Dhc	Chemical		induce		weakly			JNK	GP	activation of			NULL	MS1418 cells	0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27753_s_70	9346918	In contrast, PLA2 or PLC did not show significant induction of JNK activity, and C2-Dhc (an inactive form of ceramide) or sphingosine (a metabolic of ceramide) induces only very weak JNK activation in MS1418 cells (Fig.  6).	transcription
66907	5	336042	7	NULL	NULL	0	NULL	sphingosine	Chemical		is a metabolite of					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27753_s_70	9346918	In contrast, PLA2 or PLC did not show significant induction of JNK activity, and C2-Dhc (an inactive form of ceramide) or sphingosine (a metabolic of ceramide) induces only very weak JNK activation in MS1418 cells (Fig.  6).	transcription
66908	6	336042	7	NULL	NULL	0	NULL	sphingosine	Chemical		induce		weakly			JNK	GP	activation of			NULL	MS1418 cells	0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27753_s_70	9346918	In contrast, PLA2 or PLC did not show significant induction of JNK activity, and C2-Dhc (an inactive form of ceramide) or sphingosine (a metabolic of ceramide) induces only very weak JNK activation in MS1418 cells (Fig.  6).	transcription
60282	1	336043	5	NULL	NULL	0	NULL	sphingosine	Chemical		is converted to					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_79	10747891	To examine the possibility that sphingosine could induce apoptosis due to its conversion to ceramide, we investigated the effect of the mycotoxin fumonisin B1, a known inhibitor of ceramide synthase ( 39).	transcription
60284	2	336043	5	NULL	NULL	0	NULL	sphingosine	Chemical		induce		possibly			apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_79	10747891	To examine the possibility that sphingosine could induce apoptosis due to its conversion to ceramide, we investigated the effect of the mycotoxin fumonisin B1, a known inhibitor of ceramide synthase ( 39).	transcription
60285	3	336043	5	NULL	NULL	0	NULL	statement 1	Process		leads to					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_79	10747891	To examine the possibility that sphingosine could induce apoptosis due to its conversion to ceramide, we investigated the effect of the mycotoxin fumonisin B1, a known inhibitor of ceramide synthase ( 39).	transcription
60286	4	336043	5	NULL	NULL	0	NULL	fumonisin B1	Chemical		is a type of					mycotoxin	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_79	10747891	To examine the possibility that sphingosine could induce apoptosis due to its conversion to ceramide, we investigated the effect of the mycotoxin fumonisin B1, a known inhibitor of ceramide synthase ( 39).	transcription
60287	5	336043	5	NULL	NULL	0	NULL	fumonisin B1	Chemical		is an inhibitor of					ceramide synthase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_79	10747891	To examine the possibility that sphingosine could induce apoptosis due to its conversion to ceramide, we investigated the effect of the mycotoxin fumonisin B1, a known inhibitor of ceramide synthase ( 39).	transcription
66909	1	336043	7	NULL	NULL	0	NULL	sphingosine	Chemical		converted to					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_79	10747891	To examine the possibility that sphingosine could induce apoptosis due to its conversion to ceramide, we investigated the effect of the mycotoxin fumonisin B1, a known inhibitor of ceramide synthase ( 39).	transcription
66910	2	336043	7	NULL	NULL	0	NULL	fumonisin B1	Chemical		is an inhibitor of					ceramide synthase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_79	10747891	To examine the possibility that sphingosine could induce apoptosis due to its conversion to ceramide, we investigated the effect of the mycotoxin fumonisin B1, a known inhibitor of ceramide synthase ( 39).	transcription
66911	3	336043	7	NULL	NULL	0	NULL	fumonisin B1	Chemical		is a type of					mycotoxin	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_79	10747891	To examine the possibility that sphingosine could induce apoptosis due to its conversion to ceramide, we investigated the effect of the mycotoxin fumonisin B1, a known inhibitor of ceramide synthase ( 39).	transcription
60326	1	336044	5	NULL	NULL	0	NULL	sphingosine	Chemical		is a metabolite of					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_245	10747891	Our study also suggests a potential role for sphingosine, a further metabolite of ceramide, in Fas-induced apoptosis of type II cells, and demonstrates that similar to ceramide it also mediates cyt  c release.	transcription
60327	2	336044	5	NULL	NULL	0	NULL	apoptosis	Process		is induced by					Fas	GP				NULL	type II cells	0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_245	10747891	Our study also suggests a potential role for sphingosine, a further metabolite of ceramide, in Fas-induced apoptosis of type II cells, and demonstrates that similar to ceramide it also mediates cyt  c release.	transcription
60328	3	336044	5	NULL	NULL	0	NULL	sphingosine	Chemical		plays a role in		potentially			statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_245	10747891	Our study also suggests a potential role for sphingosine, a further metabolite of ceramide, in Fas-induced apoptosis of type II cells, and demonstrates that similar to ceramide it also mediates cyt  c release.	transcription
60329	4	336044	5	NULL	NULL	0	NULL	ceramide	Chemical		mediates					cyt c	GP	release of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_245	10747891	Our study also suggests a potential role for sphingosine, a further metabolite of ceramide, in Fas-induced apoptosis of type II cells, and demonstrates that similar to ceramide it also mediates cyt  c release.	transcription
60330	5	336044	5	NULL	NULL	0	NULL	sphingosine	Chemical		mediates					cyt c	GP	release of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_245	10747891	Our study also suggests a potential role for sphingosine, a further metabolite of ceramide, in Fas-induced apoptosis of type II cells, and demonstrates that similar to ceramide it also mediates cyt  c release.	transcription
67126	1	336044	7	NULL	NULL	0	NULL	sphingosine	Chemical		metabolite of					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_245	10747891	Our study also suggests a potential role for sphingosine, a further metabolite of ceramide, in Fas-induced apoptosis of type II cells, and demonstrates that similar to ceramide it also mediates cyt  c release.	transcription
67127	2	336044	7	NULL	NULL	NULL	NULL	sphingosine	Chemical		mediate					cyt c	GP	release of			NULL	Fas-induced apoptosis of type II cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_245	10747891	Our study also suggests a potential role for sphingosine, a further metabolite of ceramide, in Fas-induced apoptosis of type II cells, and demonstrates that similar to ceramide it also mediates cyt  c release.	transcription
67128	3	336044	7	NULL	NULL	NULL	NULL	ceramide	Chemical		mediate					cyt c	GP	release of			NULL	Fas-induced apoptosis of type II cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_245	10747891	Our study also suggests a potential role for sphingosine, a further metabolite of ceramide, in Fas-induced apoptosis of type II cells, and demonstrates that similar to ceramide it also mediates cyt  c release.	transcription
60331	1	336045	5	NULL	NULL	0	NULL	TPA	Chemical		activates					sphingosine kinase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_40_28286_s_244	10497185	Also TPA has been shown to activate sphingosine kinase, leading to increased concentrations of sphingosine-1-phosphate (SPP), which is a metabolite of ceramide and suppresses ceramide-mediated apoptosis ( 65,  77).	transcription
60332	2	336045	5	NULL	NULL	0	NULL	statement 1	Process		increases					SPP	Chemical	concentration of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_40_28286_s_244	10497185	Also TPA has been shown to activate sphingosine kinase, leading to increased concentrations of sphingosine-1-phosphate (SPP), which is a metabolite of ceramide and suppresses ceramide-mediated apoptosis ( 65,  77).	transcription
60333	3	336045	5	NULL	NULL	0	NULL	SPP	Chemical		is a metabolite of					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_40_28286_s_244	10497185	Also TPA has been shown to activate sphingosine kinase, leading to increased concentrations of sphingosine-1-phosphate (SPP), which is a metabolite of ceramide and suppresses ceramide-mediated apoptosis ( 65,  77).	transcription
60334	4	336045	5	NULL	NULL	0	NULL	apoptosis	Process		is mediated by					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_40_28286_s_244	10497185	Also TPA has been shown to activate sphingosine kinase, leading to increased concentrations of sphingosine-1-phosphate (SPP), which is a metabolite of ceramide and suppresses ceramide-mediated apoptosis ( 65,  77).	transcription
60335	5	336045	5	NULL	NULL	0	NULL	SPP	Chemical		supress					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_40_28286_s_244	10497185	Also TPA has been shown to activate sphingosine kinase, leading to increased concentrations of sphingosine-1-phosphate (SPP), which is a metabolite of ceramide and suppresses ceramide-mediated apoptosis ( 65,  77).	transcription
60336	6	336045	5	NULL	NULL	0	NULL	SPP	Chemical		is					sphingosine 1-phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_40_28286_s_244	10497185	Also TPA has been shown to activate sphingosine kinase, leading to increased concentrations of sphingosine-1-phosphate (SPP), which is a metabolite of ceramide and suppresses ceramide-mediated apoptosis ( 65,  77).	transcription
67129	1	336045	7	NULL	NULL	0	NULL	TPA	Chemical		activate					sphingosine kinase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_40_28286_s_244	10497185	Also TPA has been shown to activate sphingosine kinase, leading to increased concentrations of sphingosine-1-phosphate (SPP), which is a metabolite of ceramide and suppresses ceramide-mediated apoptosis ( 65,  77).	transcription
67130	2	336045	7	NULL	NULL	0	NULL	statement 1	Process		leads to					SPP	Chemical	increased concentrations of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_40_28286_s_244	10497185	Also TPA has been shown to activate sphingosine kinase, leading to increased concentrations of sphingosine-1-phosphate (SPP), which is a metabolite of ceramide and suppresses ceramide-mediated apoptosis ( 65,  77).	transcription
67131	3	336045	7	NULL	NULL	NULL	NULL	SPP	Chemical		is a metabolite of					ceramide	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_40_28286_s_244	10497185	Also TPA has been shown to activate sphingosine kinase, leading to increased concentrations of sphingosine-1-phosphate (SPP), which is a metabolite of ceramide and suppresses ceramide-mediated apoptosis ( 65,  77).	transcription
67132	4	336045	7	NULL	NULL	0	NULL	ceramide	Chemical		mediate					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_40_28286_s_244	10497185	Also TPA has been shown to activate sphingosine kinase, leading to increased concentrations of sphingosine-1-phosphate (SPP), which is a metabolite of ceramide and suppresses ceramide-mediated apoptosis ( 65,  77).	transcription
67133	5	336045	7	NULL	NULL	0	NULL	SPP	Chemical		suppress					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_40_28286_s_244	10497185	Also TPA has been shown to activate sphingosine kinase, leading to increased concentrations of sphingosine-1-phosphate (SPP), which is a metabolite of ceramide and suppresses ceramide-mediated apoptosis ( 65,  77).	transcription
67134	6	336045	7	NULL	NULL	0	NULL	SPP	Chemical		is					sphingosine-1-phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_40_28286_s_244	10497185	Also TPA has been shown to activate sphingosine kinase, leading to increased concentrations of sphingosine-1-phosphate (SPP), which is a metabolite of ceramide and suppresses ceramide-mediated apoptosis ( 65,  77).	transcription
60337	1	336046	5	NULL	NULL	0	NULL	sphingosine	Chemical		is produced from					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_43_30580_s_207	10521441	Such pathways could produce sphingosine from ceramide through the action of a ceramidase or utilize ceramide for ganglioside synthesis because recent studies have indicated that ganglioside synthesis is necessary for Fas-induced apoptosis ( 28).	transcription
60338	2	336046	5	NULL	NULL	0	NULL	ceramidase	GP		catalyzes					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_43_30580_s_207	10521441	Such pathways could produce sphingosine from ceramide through the action of a ceramidase or utilize ceramide for ganglioside synthesis because recent studies have indicated that ganglioside synthesis is necessary for Fas-induced apoptosis ( 28).	transcription
60339	3	336046	5	NULL	NULL	0	NULL	ganglioside	Chemical		is synthesized from					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_43_30580_s_207	10521441	Such pathways could produce sphingosine from ceramide through the action of a ceramidase or utilize ceramide for ganglioside synthesis because recent studies have indicated that ganglioside synthesis is necessary for Fas-induced apoptosis ( 28).	transcription
60340	4	336046	5	NULL	NULL	0	NULL	apoptosis	Process		is induced by					Fas	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_43_30580_s_207	10521441	Such pathways could produce sphingosine from ceramide through the action of a ceramidase or utilize ceramide for ganglioside synthesis because recent studies have indicated that ganglioside synthesis is necessary for Fas-induced apoptosis ( 28).	transcription
60341	5	336046	5	NULL	NULL	0	NULL	statement 3	Process		is required for					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_43_30580_s_207	10521441	Such pathways could produce sphingosine from ceramide through the action of a ceramidase or utilize ceramide for ganglioside synthesis because recent studies have indicated that ganglioside synthesis is necessary for Fas-induced apoptosis ( 28).	transcription
67135	1	336046	7	NULL	NULL	0	NULL	ceramide	Chemical		produced from					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_43_30580_s_207	10521441	Such pathways could produce sphingosine from ceramide through the action of a ceramidase or utilize ceramide for ganglioside synthesis because recent studies have indicated that ganglioside synthesis is necessary for Fas-induced apoptosis ( 28).	transcription
67136	2	336046	7	NULL	NULL	0	NULL	statement 1	Process		occur through					ceramidase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_43_30580_s_207	10521441	Such pathways could produce sphingosine from ceramide through the action of a ceramidase or utilize ceramide for ganglioside synthesis because recent studies have indicated that ganglioside synthesis is necessary for Fas-induced apoptosis ( 28).	transcription
67137	3	336046	7	NULL	NULL	0	NULL	ceramide	Chemical		utilized for					ganglioside synthesis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_43_30580_s_207	10521441	Such pathways could produce sphingosine from ceramide through the action of a ceramidase or utilize ceramide for ganglioside synthesis because recent studies have indicated that ganglioside synthesis is necessary for Fas-induced apoptosis ( 28).	transcription
67138	4	336046	7	NULL	NULL	0	NULL	Fas	GP		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_43_30580_s_207	10521441	Such pathways could produce sphingosine from ceramide through the action of a ceramidase or utilize ceramide for ganglioside synthesis because recent studies have indicated that ganglioside synthesis is necessary for Fas-induced apoptosis ( 28).	transcription
67139	5	336046	7	NULL	NULL	0	NULL	ganglioside synthesis	Process		necessary for					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_43_30580_s_207	10521441	Such pathways could produce sphingosine from ceramide through the action of a ceramidase or utilize ceramide for ganglioside synthesis because recent studies have indicated that ganglioside synthesis is necessary for Fas-induced apoptosis ( 28).	transcription
60425	1	336047	5	NULL	NULL	0	NULL	ceramide	Chemical		induce					apoptosis	Process				NULL	neonatal cells	0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_164	8981934	The lower effectiveness of ceramide in inducing neonatal cells into apoptosis is  in agreement with the comet data of Fig.  3 D, showing that in  adult cells, sphingosine produced a higher yield of apoptotic  type cells than did ceramide.	transcription
60427	2	336047	5	NULL	NULL	0	NULL	sphingosine	Chemical		produce					apoptotic type cells	Cell				NULL	adult cells	0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_164	8981934	The lower effectiveness of ceramide in inducing neonatal cells into apoptosis is  in agreement with the comet data of Fig.  3 D, showing that in  adult cells, sphingosine produced a higher yield of apoptotic  type cells than did ceramide.	transcription
60429	3	336047	5	NULL	NULL	0	NULL	ceramide	Chemical		produce					apoptotic type cells	Cell				NULL	adult cells	0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_164	8981934	The lower effectiveness of ceramide in inducing neonatal cells into apoptosis is  in agreement with the comet data of Fig.  3 D, showing that in  adult cells, sphingosine produced a higher yield of apoptotic  type cells than did ceramide.	transcription
60431	4	336047	5	NULL	NULL	0	NULL	statement 2	Process		higher yield than					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_164	8981934	The lower effectiveness of ceramide in inducing neonatal cells into apoptosis is  in agreement with the comet data of Fig.  3 D, showing that in  adult cells, sphingosine produced a higher yield of apoptotic  type cells than did ceramide.	transcription
67140	1	336047	7	NULL	NULL	0	NULL	neonatal cells	Cell		induced to					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_164	8981934	The lower effectiveness of ceramide in inducing neonatal cells into apoptosis is  in agreement with the comet data of Fig.  3 D, showing that in  adult cells, sphingosine produced a higher yield of apoptotic  type cells than did ceramide.	transcription
67141	2	336047	7	NULL	NULL	0	NULL	ceramide	Chemical		mediate					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_164	8981934	The lower effectiveness of ceramide in inducing neonatal cells into apoptosis is  in agreement with the comet data of Fig.  3 D, showing that in  adult cells, sphingosine produced a higher yield of apoptotic  type cells than did ceramide.	transcription
67142	3	336047	7	NULL	NULL	NULL	NULL	sphingosine	Chemical		produce					apoptotic type cells	Cell				NULL	adult cells	NULL	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_164	8981934	The lower effectiveness of ceramide in inducing neonatal cells into apoptosis is  in agreement with the comet data of Fig.  3 D, showing that in  adult cells, sphingosine produced a higher yield of apoptotic  type cells than did ceramide.	transcription
67143	4	336047	7	NULL	NULL	NULL	NULL	ceramide	Chemical		produce					apoptotic type cells	Cell				NULL	adult cells	NULL	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_164	8981934	The lower effectiveness of ceramide in inducing neonatal cells into apoptosis is  in agreement with the comet data of Fig.  3 D, showing that in  adult cells, sphingosine produced a higher yield of apoptotic  type cells than did ceramide.	transcription
67144	5	336047	7	NULL	NULL	NULL	NULL	statement 3	Process		 higher  than					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_164	8981934	The lower effectiveness of ceramide in inducing neonatal cells into apoptosis is  in agreement with the comet data of Fig.  3 D, showing that in  adult cells, sphingosine produced a higher yield of apoptotic  type cells than did ceramide.	transcription
60464	1	336048	5	NULL	NULL	0	NULL	apoptosis	Process		initiated by					TNF	GP				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_1_1_s_90	9469581	In fact, the initiation of apoptosis by TNF in some cell types appears to derive not from N-SMase-mediated generation of ceramide, but rather from the subsequent deacylation of ceramide to sphingosine  ( 46) ( 47).	transcription
60465	2	336048	5	NULL	NULL	0	NULL	ceramide	Chemical	generation of	is mediated by					N-SMase	GP				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_1_1_s_90	9469581	In fact, the initiation of apoptosis by TNF in some cell types appears to derive not from N-SMase-mediated generation of ceramide, but rather from the subsequent deacylation of ceramide to sphingosine  ( 46) ( 47).	transcription
60466	3	336048	5	NULL	NULL	0	NULL	statement 1	Process		not derived from					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_1_1_s_90	9469581	In fact, the initiation of apoptosis by TNF in some cell types appears to derive not from N-SMase-mediated generation of ceramide, but rather from the subsequent deacylation of ceramide to sphingosine  ( 46) ( 47).	transcription
60467	4	336048	5	NULL	NULL	0	NULL	ceramide	Chemical		deacetylated to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_1_1_s_90	9469581	In fact, the initiation of apoptosis by TNF in some cell types appears to derive not from N-SMase-mediated generation of ceramide, but rather from the subsequent deacylation of ceramide to sphingosine  ( 46) ( 47).	transcription
60468	5	336048	5	NULL	NULL	0	NULL	statement 2	Process		followed by					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_1_1_s_90	9469581	In fact, the initiation of apoptosis by TNF in some cell types appears to derive not from N-SMase-mediated generation of ceramide, but rather from the subsequent deacylation of ceramide to sphingosine  ( 46) ( 47).	transcription
60469	6	336048	5	NULL	NULL	0	NULL	statement 1	Process		is derived from					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_1_1_s_90	9469581	In fact, the initiation of apoptosis by TNF in some cell types appears to derive not from N-SMase-mediated generation of ceramide, but rather from the subsequent deacylation of ceramide to sphingosine  ( 46) ( 47).	transcription
67145	1	336048	7	NULL	NULL	0	NULL	TNF	GP		initiate					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_1_1_s_90	9469581	In fact, the initiation of apoptosis by TNF in some cell types appears to derive not from N-SMase-mediated generation of ceramide, but rather from the subsequent deacylation of ceramide to sphingosine  ( 46) ( 47).	transcription
67146	2	336048	7	NULL	NULL	0	NULL	N-SMase	GP		mediate					ceramide	Chemical	generation of			NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_1_1_s_90	9469581	In fact, the initiation of apoptosis by TNF in some cell types appears to derive not from N-SMase-mediated generation of ceramide, but rather from the subsequent deacylation of ceramide to sphingosine  ( 46) ( 47).	transcription
67147	3	336048	7	NULL	NULL	0	NULL	ceramide	Chemical		deacylated to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_1_1_s_90	9469581	In fact, the initiation of apoptosis by TNF in some cell types appears to derive not from N-SMase-mediated generation of ceramide, but rather from the subsequent deacylation of ceramide to sphingosine  ( 46) ( 47).	transcription
67148	4	336048	7	NULL	NULL	0	NULL	statement 1	Process		does not derive from					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_1_1_s_90	9469581	In fact, the initiation of apoptosis by TNF in some cell types appears to derive not from N-SMase-mediated generation of ceramide, but rather from the subsequent deacylation of ceramide to sphingosine  ( 46) ( 47).	transcription
67149	5	336048	7	NULL	NULL	0	NULL	statement 1	Process		derived from					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jlipidres_39_1_1_s_90	9469581	In fact, the initiation of apoptosis by TNF in some cell types appears to derive not from N-SMase-mediated generation of ceramide, but rather from the subsequent deacylation of ceramide to sphingosine  ( 46) ( 47).	transcription
60470	1	336049	5	NULL	NULL	0	NULL	sphingosine	Chemical		is converted to					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_191	9278531	This effect may be mediated by conversion of sphingosine to ceramide, because elevation of ceramide levels by treatment of PC12 cells with sphingomyelinase suppresses neurite outgrowth induced by NGF via a PKC-independent pathway (Tamura et al., 1994  ).	transcription
60471	2	336049	5	NULL	NULL	0	NULL	PC12 cells	Cell		treated with					sphingomyelinase	Chemical				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_191	9278531	This effect may be mediated by conversion of sphingosine to ceramide, because elevation of ceramide levels by treatment of PC12 cells with sphingomyelinase suppresses neurite outgrowth induced by NGF via a PKC-independent pathway (Tamura et al., 1994  ).	transcription
60472	3	336049	5	NULL	NULL	0	NULL	statement 2	Process		elevates					ceramide	Chemical	level of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_191	9278531	This effect may be mediated by conversion of sphingosine to ceramide, because elevation of ceramide levels by treatment of PC12 cells with sphingomyelinase suppresses neurite outgrowth induced by NGF via a PKC-independent pathway (Tamura et al., 1994  ).	transcription
60480	4	336049	5	NULL	NULL	0	NULL	neurite	CellComponent	outgrowth of	is induced by					NGF	GP				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_191	9278531	This effect may be mediated by conversion of sphingosine to ceramide, because elevation of ceramide levels by treatment of PC12 cells with sphingomyelinase suppresses neurite outgrowth induced by NGF via a PKC-independent pathway (Tamura et al., 1994  ).	transcription
60481	5	336049	5	NULL	NULL	0	NULL	statement 3	Process		supress					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_191	9278531	This effect may be mediated by conversion of sphingosine to ceramide, because elevation of ceramide levels by treatment of PC12 cells with sphingomyelinase suppresses neurite outgrowth induced by NGF via a PKC-independent pathway (Tamura et al., 1994  ).	transcription
60483	6	336049	5	NULL	NULL	0	NULL	statement 5	Process		via					PKC-independent pathway	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_191	9278531	This effect may be mediated by conversion of sphingosine to ceramide, because elevation of ceramide levels by treatment of PC12 cells with sphingomyelinase suppresses neurite outgrowth induced by NGF via a PKC-independent pathway (Tamura et al., 1994  ).	transcription
67150	1	336049	7	NULL	NULL	0	NULL	sphingosine	Chemical		converted to					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_191	9278531	This effect may be mediated by conversion of sphingosine to ceramide, because elevation of ceramide levels by treatment of PC12 cells with sphingomyelinase suppresses neurite outgrowth induced by NGF via a PKC-independent pathway (Tamura et al., 1994  ).	transcription
67151	2	336049	7	NULL	NULL	0	NULL	PC12 cells 	Cell		treated with					sphingomyelinase	GP				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_191	9278531	This effect may be mediated by conversion of sphingosine to ceramide, because elevation of ceramide levels by treatment of PC12 cells with sphingomyelinase suppresses neurite outgrowth induced by NGF via a PKC-independent pathway (Tamura et al., 1994  ).	transcription
67152	3	336049	7	NULL	NULL	0	NULL	statement 2	Process		elevates					ceramide	Chemical	levels of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_191	9278531	This effect may be mediated by conversion of sphingosine to ceramide, because elevation of ceramide levels by treatment of PC12 cells with sphingomyelinase suppresses neurite outgrowth induced by NGF via a PKC-independent pathway (Tamura et al., 1994  ).	transcription
67153	4	336049	7	NULL	NULL	0	NULL	NGF	GP		induce					neurite outgrowth	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_191	9278531	This effect may be mediated by conversion of sphingosine to ceramide, because elevation of ceramide levels by treatment of PC12 cells with sphingomyelinase suppresses neurite outgrowth induced by NGF via a PKC-independent pathway (Tamura et al., 1994  ).	transcription
67154	5	336049	7	NULL	NULL	0	NULL	statement 3	Process		suppress					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_191	9278531	This effect may be mediated by conversion of sphingosine to ceramide, because elevation of ceramide levels by treatment of PC12 cells with sphingomyelinase suppresses neurite outgrowth induced by NGF via a PKC-independent pathway (Tamura et al., 1994  ).	transcription
67155	6	336049	7	NULL	NULL	0	NULL	statement 4	Process		via					PKC-independent pathway	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_191	9278531	This effect may be mediated by conversion of sphingosine to ceramide, because elevation of ceramide levels by treatment of PC12 cells with sphingomyelinase suppresses neurite outgrowth induced by NGF via a PKC-independent pathway (Tamura et al., 1994  ).	transcription
60484	1	336050	5	NULL	NULL	0	NULL	PKC	GP	activation of	is dependent on					DAG	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_221	9536027	Studies show that DAG-dependent PKC activation and ceramide production have an antagonistic relationship, and sphinganine and sphingosine inhibit PKC, thereby increasing the potency and efficacy of the ceramide in inducing apoptosis in cell lines (Jarvis  et al., 1996  ).	transcription
60485	2	336050	5	NULL	NULL	0	NULL	statement 1	Process		is antagonistic to					ceramide	Chemical	production of			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_221	9536027	Studies show that DAG-dependent PKC activation and ceramide production have an antagonistic relationship, and sphinganine and sphingosine inhibit PKC, thereby increasing the potency and efficacy of the ceramide in inducing apoptosis in cell lines (Jarvis  et al., 1996  ).	transcription
60487	3	336050	5	NULL	NULL	0	NULL	sphinganine	Chemical		inhibits					PKC	GP				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_221	9536027	Studies show that DAG-dependent PKC activation and ceramide production have an antagonistic relationship, and sphinganine and sphingosine inhibit PKC, thereby increasing the potency and efficacy of the ceramide in inducing apoptosis in cell lines (Jarvis  et al., 1996  ).	transcription
60488	4	336050	5	NULL	NULL	0	NULL	sphingosine	Chemical		inhibits					PKC	GP				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_221	9536027	Studies show that DAG-dependent PKC activation and ceramide production have an antagonistic relationship, and sphinganine and sphingosine inhibit PKC, thereby increasing the potency and efficacy of the ceramide in inducing apoptosis in cell lines (Jarvis  et al., 1996  ).	transcription
60489	5	336050	5	NULL	NULL	0	NULL	ceramide	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_221	9536027	Studies show that DAG-dependent PKC activation and ceramide production have an antagonistic relationship, and sphinganine and sphingosine inhibit PKC, thereby increasing the potency and efficacy of the ceramide in inducing apoptosis in cell lines (Jarvis  et al., 1996  ).	transcription
60491	6	336050	5	NULL	NULL	0	NULL	statement 3	Process		increases					statement 5	Process	potency of			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_221	9536027	Studies show that DAG-dependent PKC activation and ceramide production have an antagonistic relationship, and sphinganine and sphingosine inhibit PKC, thereby increasing the potency and efficacy of the ceramide in inducing apoptosis in cell lines (Jarvis  et al., 1996  ).	transcription
60493	7	336050	5	NULL	NULL	0	NULL	statement 3	Process		increases					statement 5	Process	efficacy of			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_221	9536027	Studies show that DAG-dependent PKC activation and ceramide production have an antagonistic relationship, and sphinganine and sphingosine inhibit PKC, thereby increasing the potency and efficacy of the ceramide in inducing apoptosis in cell lines (Jarvis  et al., 1996  ).	transcription
60494	8	336050	5	NULL	NULL	0	NULL	statement 4	Process		increases					statement 5	Process	potency of			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_221	9536027	Studies show that DAG-dependent PKC activation and ceramide production have an antagonistic relationship, and sphinganine and sphingosine inhibit PKC, thereby increasing the potency and efficacy of the ceramide in inducing apoptosis in cell lines (Jarvis  et al., 1996  ).	transcription
60495	9	336050	5	NULL	NULL	0	NULL	statement 4	Process		increases					statement 5	Process	efficacy of			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_221	9536027	Studies show that DAG-dependent PKC activation and ceramide production have an antagonistic relationship, and sphinganine and sphingosine inhibit PKC, thereby increasing the potency and efficacy of the ceramide in inducing apoptosis in cell lines (Jarvis  et al., 1996  ).	transcription
67156	1	336050	7	NULL	NULL	0	NULL	PKC	GP	activation of	depends on					DAG	Chemical				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_221	9536027	Studies show that DAG-dependent PKC activation and ceramide production have an antagonistic relationship, and sphinganine and sphingosine inhibit PKC, thereby increasing the potency and efficacy of the ceramide in inducing apoptosis in cell lines (Jarvis  et al., 1996  ).	transcription
67157	2	336050	7	NULL	NULL	0	NULL	ceramide	Chemical	production of	depends on					DAG	Chemical				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_221	9536027	Studies show that DAG-dependent PKC activation and ceramide production have an antagonistic relationship, and sphinganine and sphingosine inhibit PKC, thereby increasing the potency and efficacy of the ceramide in inducing apoptosis in cell lines (Jarvis  et al., 1996  ).	transcription
67158	3	336050	7	NULL	NULL	0	NULL	statement 1	Process		antagonizes with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_221	9536027	Studies show that DAG-dependent PKC activation and ceramide production have an antagonistic relationship, and sphinganine and sphingosine inhibit PKC, thereby increasing the potency and efficacy of the ceramide in inducing apoptosis in cell lines (Jarvis  et al., 1996  ).	transcription
67159	4	336050	7	NULL	NULL	0	NULL	sphinganine	Chemical		inhibit					PKC	GP				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_221	9536027	Studies show that DAG-dependent PKC activation and ceramide production have an antagonistic relationship, and sphinganine and sphingosine inhibit PKC, thereby increasing the potency and efficacy of the ceramide in inducing apoptosis in cell lines (Jarvis  et al., 1996  ).	transcription
67160	5	336050	7	NULL	NULL	0	NULL	sphingosine	Chemical		inhibit					PKC	GP				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_221	9536027	Studies show that DAG-dependent PKC activation and ceramide production have an antagonistic relationship, and sphinganine and sphingosine inhibit PKC, thereby increasing the potency and efficacy of the ceramide in inducing apoptosis in cell lines (Jarvis  et al., 1996  ).	transcription
67161	6	336050	7	NULL	NULL	NULL	NULL	statement 4	Process		increase					ceramide	Chemical	potency of;;efficacy of			NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_221	9536027	Studies show that DAG-dependent PKC activation and ceramide production have an antagonistic relationship, and sphinganine and sphingosine inhibit PKC, thereby increasing the potency and efficacy of the ceramide in inducing apoptosis in cell lines (Jarvis  et al., 1996  ).	transcription
67162	7	336050	7	NULL	NULL	NULL	NULL	statement 5	Process		increase					ceramide	Chemical	potency of;;efficacy of			NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_221	9536027	Studies show that DAG-dependent PKC activation and ceramide production have an antagonistic relationship, and sphinganine and sphingosine inhibit PKC, thereby increasing the potency and efficacy of the ceramide in inducing apoptosis in cell lines (Jarvis  et al., 1996  ).	transcription
67163	8	336050	7	NULL	NULL	0	NULL	statement 6	Process		induce					apoptosis	Process				NULL	cell lines	0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_221	9536027	Studies show that DAG-dependent PKC activation and ceramide production have an antagonistic relationship, and sphinganine and sphingosine inhibit PKC, thereby increasing the potency and efficacy of the ceramide in inducing apoptosis in cell lines (Jarvis  et al., 1996  ).	transcription
67164	9	336050	7	NULL	NULL	0	NULL	statement 7	Process		induce					apoptosis	Process				NULL	cell lines	0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_221	9536027	Studies show that DAG-dependent PKC activation and ceramide production have an antagonistic relationship, and sphinganine and sphingosine inhibit PKC, thereby increasing the potency and efficacy of the ceramide in inducing apoptosis in cell lines (Jarvis  et al., 1996  ).	transcription
60497	1	336051	5	NULL	NULL	0	NULL	inflammatory cytokines	GP		stimulates					sphingomyelinase	GP				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_ann-n-y-acad-sci_845_1_9668339_s_5	9668339	Inflammatory cytokines stimulate sphingomyelinase,  but not ceramidase, leading to accumulation of ceramide, whereas growth  signals also leading to accumulation of ceramide, whereas growth signals  also stimulate ceramidase and sphingosine kinase leading to increased  SPP levels.	transcription
60498	2	336051	5	NULL	NULL	0	NULL	inflammatory cytokines	GP		does not stimulate					ceramidase	GP				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_ann-n-y-acad-sci_845_1_9668339_s_5	9668339	Inflammatory cytokines stimulate sphingomyelinase,  but not ceramidase, leading to accumulation of ceramide, whereas growth  signals also leading to accumulation of ceramide, whereas growth signals  also stimulate ceramidase and sphingosine kinase leading to increased  SPP levels.	transcription
60499	3	336051	5	NULL	NULL	0	NULL	statement 2	Process		leads to					ceramide	Chemical	accumulation of			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_ann-n-y-acad-sci_845_1_9668339_s_5	9668339	Inflammatory cytokines stimulate sphingomyelinase,  but not ceramidase, leading to accumulation of ceramide, whereas growth  signals also leading to accumulation of ceramide, whereas growth signals  also stimulate ceramidase and sphingosine kinase leading to increased  SPP levels.	transcription
60657	4	336051	5	NULL	NULL	0	NULL	growth signals	GP		accumulates					ceramide	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_ann-n-y-acad-sci_845_1_9668339_s_5	9668339	Inflammatory cytokines stimulate sphingomyelinase,  but not ceramidase, leading to accumulation of ceramide, whereas growth  signals also leading to accumulation of ceramide, whereas growth signals  also stimulate ceramidase and sphingosine kinase leading to increased  SPP levels.	transcription
60658	5	336051	5	NULL	NULL	0	NULL	growth signals	GP		stimulates					ceramidase	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_ann-n-y-acad-sci_845_1_9668339_s_5	9668339	Inflammatory cytokines stimulate sphingomyelinase,  but not ceramidase, leading to accumulation of ceramide, whereas growth  signals also leading to accumulation of ceramide, whereas growth signals  also stimulate ceramidase and sphingosine kinase leading to increased  SPP levels.	transcription
60659	6	336051	5	NULL	NULL	0	NULL	growth signals	GP		stimulates					sphingosine kinase	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_ann-n-y-acad-sci_845_1_9668339_s_5	9668339	Inflammatory cytokines stimulate sphingomyelinase,  but not ceramidase, leading to accumulation of ceramide, whereas growth  signals also leading to accumulation of ceramide, whereas growth signals  also stimulate ceramidase and sphingosine kinase leading to increased  SPP levels.	transcription
60660	7	336051	5	NULL	NULL	0	NULL	statement 5	Process		increases					SPP	Chemical	level of			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_ann-n-y-acad-sci_845_1_9668339_s_5	9668339	Inflammatory cytokines stimulate sphingomyelinase,  but not ceramidase, leading to accumulation of ceramide, whereas growth  signals also leading to accumulation of ceramide, whereas growth signals  also stimulate ceramidase and sphingosine kinase leading to increased  SPP levels.	transcription
60661	8	336051	5	NULL	NULL	0	NULL	statement 6	Process		increases					SPP	Chemical	level of			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_ann-n-y-acad-sci_845_1_9668339_s_5	9668339	Inflammatory cytokines stimulate sphingomyelinase,  but not ceramidase, leading to accumulation of ceramide, whereas growth  signals also leading to accumulation of ceramide, whereas growth signals  also stimulate ceramidase and sphingosine kinase leading to increased  SPP levels.	transcription
67165	1	336051	7	NULL	NULL	NULL	NULL	Inflammatory cytokines	GP		stimulate					sphingomyelinase	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_ann-n-y-acad-sci_845_1_9668339_s_5	9668339	Inflammatory cytokines stimulate sphingomyelinase,  but not ceramidase, leading to accumulation of ceramide, whereas growth  signals also leading to accumulation of ceramide, whereas growth signals  also stimulate ceramidase and sphingosine kinase leading to increased  SPP levels.	transcription
67166	2	336051	7	NULL	NULL	0	NULL	Inflammatory cytokines 	GP		does not stimulate					ceramidase	GP				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_ann-n-y-acad-sci_845_1_9668339_s_5	9668339	Inflammatory cytokines stimulate sphingomyelinase,  but not ceramidase, leading to accumulation of ceramide, whereas growth  signals also leading to accumulation of ceramide, whereas growth signals  also stimulate ceramidase and sphingosine kinase leading to increased  SPP levels.	transcription
67167	3	336051	7	NULL	NULL	0	NULL	statement 2	Process		leads to					ceramide	Chemical	accumulation of			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_ann-n-y-acad-sci_845_1_9668339_s_5	9668339	Inflammatory cytokines stimulate sphingomyelinase,  but not ceramidase, leading to accumulation of ceramide, whereas growth  signals also leading to accumulation of ceramide, whereas growth signals  also stimulate ceramidase and sphingosine kinase leading to increased  SPP levels.	transcription
67168	4	336051	7	NULL	NULL	NULL	NULL	growth signals	GP		leads to					ceramide	Chemical	accumulation of			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_ann-n-y-acad-sci_845_1_9668339_s_5	9668339	Inflammatory cytokines stimulate sphingomyelinase,  but not ceramidase, leading to accumulation of ceramide, whereas growth  signals also leading to accumulation of ceramide, whereas growth signals  also stimulate ceramidase and sphingosine kinase leading to increased  SPP levels.	transcription
67169	5	336051	7	NULL	NULL	0	NULL	growth signals	GP		stimulate					ceramidase	GP				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_ann-n-y-acad-sci_845_1_9668339_s_5	9668339	Inflammatory cytokines stimulate sphingomyelinase,  but not ceramidase, leading to accumulation of ceramide, whereas growth  signals also leading to accumulation of ceramide, whereas growth signals  also stimulate ceramidase and sphingosine kinase leading to increased  SPP levels.	transcription
67170	6	336051	7	NULL	NULL	NULL	NULL	growth signals	GP		stimulate					sphingosine kinase	GP				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_ann-n-y-acad-sci_845_1_9668339_s_5	9668339	Inflammatory cytokines stimulate sphingomyelinase,  but not ceramidase, leading to accumulation of ceramide, whereas growth  signals also leading to accumulation of ceramide, whereas growth signals  also stimulate ceramidase and sphingosine kinase leading to increased  SPP levels.	transcription
67171	7	336051	7	NULL	NULL	0	NULL	statement 5	Process		leads to					SPP	Chemical	increased levels of			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_ann-n-y-acad-sci_845_1_9668339_s_5	9668339	Inflammatory cytokines stimulate sphingomyelinase,  but not ceramidase, leading to accumulation of ceramide, whereas growth  signals also leading to accumulation of ceramide, whereas growth signals  also stimulate ceramidase and sphingosine kinase leading to increased  SPP levels.	transcription
67172	8	336051	7	NULL	NULL	0	NULL	statement 6	Process		leads to					SPP	Chemical	increased levels of			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_ann-n-y-acad-sci_845_1_9668339_s_5	9668339	Inflammatory cytokines stimulate sphingomyelinase,  but not ceramidase, leading to accumulation of ceramide, whereas growth  signals also leading to accumulation of ceramide, whereas growth signals  also stimulate ceramidase and sphingosine kinase leading to increased  SPP levels.	transcription
60662	1	336052	5	NULL	NULL	0	NULL	HeLa cells	Cell		treated with					D-e-sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_3_1555_s_269	15647381	In contrast, treatment of HeLa cells with 2.5 muM D-e-sphingosine in the presence of 50 muM fumonisin B1 (FB1), which prevents sphingosine from being incorporated into ceramide by inhibiting ceramide synthase, rapidly induced the GC fragmentation ( Figure 9E).	transcription
60663	2	336052	5	NULL	NULL	0	NULL	statement 1	Process		in the presence of					FB1	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_3_1555_s_269	15647381	In contrast, treatment of HeLa cells with 2.5 muM D-e-sphingosine in the presence of 50 muM fumonisin B1 (FB1), which prevents sphingosine from being incorporated into ceramide by inhibiting ceramide synthase, rapidly induced the GC fragmentation ( Figure 9E).	transcription
60664	3	336052	5	NULL	NULL	0	NULL	FB1	Chemical		is					fumonisin B1	Chemical				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_3_1555_s_269	15647381	In contrast, treatment of HeLa cells with 2.5 muM D-e-sphingosine in the presence of 50 muM fumonisin B1 (FB1), which prevents sphingosine from being incorporated into ceramide by inhibiting ceramide synthase, rapidly induced the GC fragmentation ( Figure 9E).	transcription
60665	4	336052	5	NULL	NULL	0	NULL	sphingosine	Chemical		is incorporated into					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_3_1555_s_269	15647381	In contrast, treatment of HeLa cells with 2.5 muM D-e-sphingosine in the presence of 50 muM fumonisin B1 (FB1), which prevents sphingosine from being incorporated into ceramide by inhibiting ceramide synthase, rapidly induced the GC fragmentation ( Figure 9E).	transcription
60666	5	336052	5	NULL	NULL	0	NULL	ceramide synthase	GP		plays a role in					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_3_1555_s_269	15647381	In contrast, treatment of HeLa cells with 2.5 muM D-e-sphingosine in the presence of 50 muM fumonisin B1 (FB1), which prevents sphingosine from being incorporated into ceramide by inhibiting ceramide synthase, rapidly induced the GC fragmentation ( Figure 9E).	transcription
60667	6	336052	5	NULL	NULL	0	NULL	FB1	Chemical		inhibits					ceramide synthase	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_3_1555_s_269	15647381	In contrast, treatment of HeLa cells with 2.5 muM D-e-sphingosine in the presence of 50 muM fumonisin B1 (FB1), which prevents sphingosine from being incorporated into ceramide by inhibiting ceramide synthase, rapidly induced the GC fragmentation ( Figure 9E).	transcription
60668	7	336052	5	NULL	NULL	0	NULL	statement 6	Process		inhibits					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_3_1555_s_269	15647381	In contrast, treatment of HeLa cells with 2.5 muM D-e-sphingosine in the presence of 50 muM fumonisin B1 (FB1), which prevents sphingosine from being incorporated into ceramide by inhibiting ceramide synthase, rapidly induced the GC fragmentation ( Figure 9E).	transcription
60669	8	336052	5	NULL	NULL	0	NULL	statement 1	Process		induces					GC	CellComponent	fragmentation of			NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_3_1555_s_269	15647381	In contrast, treatment of HeLa cells with 2.5 muM D-e-sphingosine in the presence of 50 muM fumonisin B1 (FB1), which prevents sphingosine from being incorporated into ceramide by inhibiting ceramide synthase, rapidly induced the GC fragmentation ( Figure 9E).	transcription
67175	1	336052	7	NULL	NULL	NULL	NULL	FB1	Chemical		is					fumonisin B1	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_3_1555_s_269	15647381	In contrast, treatment of HeLa cells with 2.5 muM D-e-sphingosine in the presence of 50 muM fumonisin B1 (FB1), which prevents sphingosine from being incorporated into ceramide by inhibiting ceramide synthase, rapidly induced the GC fragmentation ( Figure 9E).	transcription
67176	2	336052	7	NULL	NULL	NULL	NULL	sphingosine	Chemical		incorporated into					ceramide	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_3_1555_s_269	15647381	In contrast, treatment of HeLa cells with 2.5 muM D-e-sphingosine in the presence of 50 muM fumonisin B1 (FB1), which prevents sphingosine from being incorporated into ceramide by inhibiting ceramide synthase, rapidly induced the GC fragmentation ( Figure 9E).	transcription
67177	3	336052	7	NULL	NULL	NULL	NULL	ceramide synthase	GP		mediate					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_3_1555_s_269	15647381	In contrast, treatment of HeLa cells with 2.5 muM D-e-sphingosine in the presence of 50 muM fumonisin B1 (FB1), which prevents sphingosine from being incorporated into ceramide by inhibiting ceramide synthase, rapidly induced the GC fragmentation ( Figure 9E).	transcription
67178	4	336052	7	NULL	NULL	NULL	NULL	FB1	Chemical		inhibit					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_3_1555_s_269	15647381	In contrast, treatment of HeLa cells with 2.5 muM D-e-sphingosine in the presence of 50 muM fumonisin B1 (FB1), which prevents sphingosine from being incorporated into ceramide by inhibiting ceramide synthase, rapidly induced the GC fragmentation ( Figure 9E).	transcription
67179	5	336052	7	NULL	NULL	0	NULL	FB1	Chemical		induce		rapidly			GC fragmentation	Process				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_3_1555_s_269	15647381	In contrast, treatment of HeLa cells with 2.5 muM D-e-sphingosine in the presence of 50 muM fumonisin B1 (FB1), which prevents sphingosine from being incorporated into ceramide by inhibiting ceramide synthase, rapidly induced the GC fragmentation ( Figure 9E).	transcription
60670	1	336053	5	NULL	NULL	0	NULL	CDase	GP	guinea pig;;epidermis	suppressed by					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_21_12677_s_151	7759519	The fact that two CDase species in guinea pig epidermis  were suppressed by the sphingosine ( Fig. 7) suggests that  ceramide hydrolysis liberating free sphingosine could also provide a  feedback mechanism for regulating ceramide breakdown, supporting the  notion that CDase activities are controlled by the balance of substrate  degradation and production.	transcription
60671	2	336053	5	NULL	NULL	0	NULL	ceramide	Chemical	hydrolysis of	liberates					sphingosine	Chemical	free			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_21_12677_s_151	7759519	The fact that two CDase species in guinea pig epidermis  were suppressed by the sphingosine ( Fig. 7) suggests that  ceramide hydrolysis liberating free sphingosine could also provide a  feedback mechanism for regulating ceramide breakdown, supporting the  notion that CDase activities are controlled by the balance of substrate  degradation and production.	transcription
60672	3	336053	5	NULL	NULL	0	NULL	statement 2	Process		regulates					ceramide	Chemical	breakdown of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_21_12677_s_151	7759519	The fact that two CDase species in guinea pig epidermis  were suppressed by the sphingosine ( Fig. 7) suggests that  ceramide hydrolysis liberating free sphingosine could also provide a  feedback mechanism for regulating ceramide breakdown, supporting the  notion that CDase activities are controlled by the balance of substrate  degradation and production.	transcription
60673	4	336053	5	NULL	NULL	0	NULL	statement 3	Process		is a type of					feedback mechanism	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_21_12677_s_151	7759519	The fact that two CDase species in guinea pig epidermis  were suppressed by the sphingosine ( Fig. 7) suggests that  ceramide hydrolysis liberating free sphingosine could also provide a  feedback mechanism for regulating ceramide breakdown, supporting the  notion that CDase activities are controlled by the balance of substrate  degradation and production.	transcription
67180	1	336053	7	NULL	NULL	0	NULL	sphingosine	Chemical		suppress					 CDase	GP	guinea pig epidermis			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_21_12677_s_151	7759519	The fact that two CDase species in guinea pig epidermis  were suppressed by the sphingosine ( Fig. 7) suggests that  ceramide hydrolysis liberating free sphingosine could also provide a  feedback mechanism for regulating ceramide breakdown, supporting the  notion that CDase activities are controlled by the balance of substrate  degradation and production.	transcription
67181	2	336053	7	NULL	NULL	0	NULL	ceramide	Chemical		hydrolyzed to					sphingosine	Chemical	liberate free			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_21_12677_s_151	7759519	The fact that two CDase species in guinea pig epidermis  were suppressed by the sphingosine ( Fig. 7) suggests that  ceramide hydrolysis liberating free sphingosine could also provide a  feedback mechanism for regulating ceramide breakdown, supporting the  notion that CDase activities are controlled by the balance of substrate  degradation and production.	transcription
67182	3	336053	7	NULL	NULL	0	NULL	statement 2	Process		regulate					ceramide	Chemical	breakdown of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_21_12677_s_151	7759519	The fact that two CDase species in guinea pig epidermis  were suppressed by the sphingosine ( Fig. 7) suggests that  ceramide hydrolysis liberating free sphingosine could also provide a  feedback mechanism for regulating ceramide breakdown, supporting the  notion that CDase activities are controlled by the balance of substrate  degradation and production.	transcription
60674	1	336054	5	NULL	NULL	0	NULL	N-SMase	GP		is					neutral sphingomyelinase	GP				NULL		0	NULL	NULL	NULL	gw70_circulation_109_3_406_s_21	14732751	7,8  We proposed that sphingosine was produced by downstream ceramide production after activation by arachidonic acid of the Mg-dependent neutral sphingomyelinase (N-SMase).	transcription
60675	2	336054	5	NULL	NULL	0	NULL	N-SMase	GP		is dependent on					Mg	Chemical				NULL		0	NULL	NULL	NULL	gw70_circulation_109_3_406_s_21	14732751	7,8  We proposed that sphingosine was produced by downstream ceramide production after activation by arachidonic acid of the Mg-dependent neutral sphingomyelinase (N-SMase).	transcription
60676	3	336054	5	NULL	NULL	0	NULL	arachidonic acid	Chemical		activates					statement 2	GP				NULL		0	NULL	NULL	NULL	gw70_circulation_109_3_406_s_21	14732751	7,8  We proposed that sphingosine was produced by downstream ceramide production after activation by arachidonic acid of the Mg-dependent neutral sphingomyelinase (N-SMase).	transcription
60677	4	336054	5	NULL	NULL	0	NULL	statement 3	Process		produce					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw70_circulation_109_3_406_s_21	14732751	7,8  We proposed that sphingosine was produced by downstream ceramide production after activation by arachidonic acid of the Mg-dependent neutral sphingomyelinase (N-SMase).	transcription
60678	5	336054	5	NULL	NULL	0	NULL	statement 4	Process		produce					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_circulation_109_3_406_s_21	14732751	7,8  We proposed that sphingosine was produced by downstream ceramide production after activation by arachidonic acid of the Mg-dependent neutral sphingomyelinase (N-SMase).	transcription
67183	1	336054	7	NULL	NULL	0	NULL	arachidonic acid	Chemical		activate					N-SMase	GP				NULL		0	NULL	NULL	NULL	gw70_circulation_109_3_406_s_21	14732751	7,8  We proposed that sphingosine was produced by downstream ceramide production after activation by arachidonic acid of the Mg-dependent neutral sphingomyelinase (N-SMase).	transcription
67184	2	336054	7	NULL	NULL	0	NULL	sphingosine 	Chemical		produced by					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw70_circulation_109_3_406_s_21	14732751	7,8  We proposed that sphingosine was produced by downstream ceramide production after activation by arachidonic acid of the Mg-dependent neutral sphingomyelinase (N-SMase).	transcription
67185	3	336054	7	NULL	NULL	0	NULL	statement 2	Process		occur after					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_circulation_109_3_406_s_21	14732751	7,8  We proposed that sphingosine was produced by downstream ceramide production after activation by arachidonic acid of the Mg-dependent neutral sphingomyelinase (N-SMase).	transcription
67186	4	336054	7	NULL	NULL	0	NULL	N-SMase	GP		is					neutral sphingomyelinase	GP				NULL		0	NULL	NULL	NULL	gw70_circulation_109_3_406_s_21	14732751	7,8  We proposed that sphingosine was produced by downstream ceramide production after activation by arachidonic acid of the Mg-dependent neutral sphingomyelinase (N-SMase).	transcription
60679	1	336055	5	NULL	NULL	0	NULL	TNF-alpha	GP		is a type of					cytokine	GP				NULL		0	NULL	NULL	NULL	gw70_circulationres_95_12_1140_s_103	15591236	Cytokines such as TNF-alpha also deplete GSH and activate membrane-associated neutral sphingomyelinase (NSM),  which in turn increases ceramide (C) and sphingosine levels.	transcription
60680	2	336055	5	NULL	NULL	0	NULL	TNF-alpha	GP		deplete					GSH	GP				NULL		0	NULL	NULL	NULL	gw70_circulationres_95_12_1140_s_103	15591236	Cytokines such as TNF-alpha also deplete GSH and activate membrane-associated neutral sphingomyelinase (NSM),  which in turn increases ceramide (C) and sphingosine levels.	transcription
60681	3	336055	5	NULL	NULL	0	NULL	TNF-alpha	GP		activates					NSM	GP				NULL		0	NULL	NULL	NULL	gw70_circulationres_95_12_1140_s_103	15591236	Cytokines such as TNF-alpha also deplete GSH and activate membrane-associated neutral sphingomyelinase (NSM),  which in turn increases ceramide (C) and sphingosine levels.	transcription
60682	4	336055	5	NULL	NULL	0	NULL	statement 3	Process		increases					ceramide	Chemical	level of			NULL		0	NULL	NULL	NULL	gw70_circulationres_95_12_1140_s_103	15591236	Cytokines such as TNF-alpha also deplete GSH and activate membrane-associated neutral sphingomyelinase (NSM),  which in turn increases ceramide (C) and sphingosine levels.	transcription
60683	5	336055	5	NULL	NULL	0	NULL	statement 3	Process		increases					sphingosine	Chemical	level of			NULL		0	NULL	NULL	NULL	gw70_circulationres_95_12_1140_s_103	15591236	Cytokines such as TNF-alpha also deplete GSH and activate membrane-associated neutral sphingomyelinase (NSM),  which in turn increases ceramide (C) and sphingosine levels.	transcription
60684	6	336055	5	NULL	NULL	0	NULL	NSM	GP		is					neutral sphingomyelinase	GP				NULL		0	NULL	NULL	NULL	gw70_circulationres_95_12_1140_s_103	15591236	Cytokines such as TNF-alpha also deplete GSH and activate membrane-associated neutral sphingomyelinase (NSM),  which in turn increases ceramide (C) and sphingosine levels.	transcription
60685	7	336055	5	NULL	NULL	0	NULL	NSM	GP		is associated with					membrane	CellComponent				NULL		0	NULL	NULL	NULL	gw70_circulationres_95_12_1140_s_103	15591236	Cytokines such as TNF-alpha also deplete GSH and activate membrane-associated neutral sphingomyelinase (NSM),  which in turn increases ceramide (C) and sphingosine levels.	transcription
67187	1	336055	7	NULL	NULL	0	NULL	TNF-alpha	GP		deplete					GSH	GP				NULL		0	NULL	NULL	NULL	gw70_circulationres_95_12_1140_s_103	15591236	Cytokines such as TNF-alpha also deplete GSH and activate membrane-associated neutral sphingomyelinase (NSM),  which in turn increases ceramide (C) and sphingosine levels.	transcription
67188	2	336055	7	NULL	NULL	NULL	NULL	TNF-alpha	GP		activate					NSM	GP	membrane-associated			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_12_1140_s_103	15591236	Cytokines such as TNF-alpha also deplete GSH and activate membrane-associated neutral sphingomyelinase (NSM),  which in turn increases ceramide (C) and sphingosine levels.	transcription
67189	3	336055	7	NULL	NULL	0	NULL	statement 1	Process		leads to					ceramide	Chemical	increased levels of			NULL		0	NULL	NULL	NULL	gw70_circulationres_95_12_1140_s_103	15591236	Cytokines such as TNF-alpha also deplete GSH and activate membrane-associated neutral sphingomyelinase (NSM),  which in turn increases ceramide (C) and sphingosine levels.	transcription
67190	4	336055	7	NULL	NULL	0	NULL	statement 2	Process		leads to					ceramide	Chemical	increased levels of			NULL		0	NULL	NULL	NULL	gw70_circulationres_95_12_1140_s_103	15591236	Cytokines such as TNF-alpha also deplete GSH and activate membrane-associated neutral sphingomyelinase (NSM),  which in turn increases ceramide (C) and sphingosine levels.	transcription
67191	5	336055	7	NULL	NULL	NULL	NULL	statement 1	Process		leads to					sphingosine	Chemical	increased levels of			NULL		NULL	NULL	NULL	NULL	gw70_circulationres_95_12_1140_s_103	15591236	Cytokines such as TNF-alpha also deplete GSH and activate membrane-associated neutral sphingomyelinase (NSM),  which in turn increases ceramide (C) and sphingosine levels.	transcription
67192	6	336055	7	NULL	NULL	0	NULL	statement 2	Process		leads to					sphingosine	Chemical	increased levels of			NULL		0	NULL	NULL	NULL	gw70_circulationres_95_12_1140_s_103	15591236	Cytokines such as TNF-alpha also deplete GSH and activate membrane-associated neutral sphingomyelinase (NSM),  which in turn increases ceramide (C) and sphingosine levels.	transcription
67193	7	336055	7	NULL	NULL	0	NULL	NSM	GP		is					neutral sphingomyelinase	GP				NULL		0	NULL	NULL	NULL	gw70_circulationres_95_12_1140_s_103	15591236	Cytokines such as TNF-alpha also deplete GSH and activate membrane-associated neutral sphingomyelinase (NSM),  which in turn increases ceramide (C) and sphingosine levels.	transcription
60686	1	336056	5	NULL	NULL	0	NULL	ceramide	Chemical		induce					neuro-protection	Process				NULL		0	NULL	NULL	NULL	gw70_neuropharmacology_45_8_1130_s_300	14614956	We assessed the effects of the ceramidase  inhibitor NOE and the sphingosine kinase inhibitor DMS ( [  Edsall et al., 1998]) on ceramide-induced neuro-protection.	transcription
60687	2	336056	5	NULL	NULL	0	NULL	NOE	Chemical		is an inhibitor of					ceramidase	GP				NULL		0	NULL	NULL	NULL	gw70_neuropharmacology_45_8_1130_s_300	14614956	We assessed the effects of the ceramidase  inhibitor NOE and the sphingosine kinase inhibitor DMS ( [  Edsall et al., 1998]) on ceramide-induced neuro-protection.	transcription
60688	3	336056	5	NULL	NULL	0	NULL	DMS	Chemical		is an inhibitor of					sphingosine kinase	GP				NULL		0	NULL	NULL	NULL	gw70_neuropharmacology_45_8_1130_s_300	14614956	We assessed the effects of the ceramidase  inhibitor NOE and the sphingosine kinase inhibitor DMS ( [  Edsall et al., 1998]) on ceramide-induced neuro-protection.	transcription
60689	4	336056	5	NULL	NULL	0	NULL	NOE	Chemical		effects		potentially			statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_neuropharmacology_45_8_1130_s_300	14614956	We assessed the effects of the ceramidase  inhibitor NOE and the sphingosine kinase inhibitor DMS ( [  Edsall et al., 1998]) on ceramide-induced neuro-protection.	transcription
60690	5	336056	5	NULL	NULL	0	NULL	DMS	Chemical		effects		potentially			statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_neuropharmacology_45_8_1130_s_300	14614956	We assessed the effects of the ceramidase  inhibitor NOE and the sphingosine kinase inhibitor DMS ( [  Edsall et al., 1998]) on ceramide-induced neuro-protection.	transcription
67408	1	336056	7	NULL	NULL	0	NULL	ceramide 	Chemical		induce					 neuro-protection	Process				NULL		0	NULL	NULL	NULL	gw70_neuropharmacology_45_8_1130_s_300	14614956	We assessed the effects of the ceramidase  inhibitor NOE and the sphingosine kinase inhibitor DMS ( [  Edsall et al., 1998]) on ceramide-induced neuro-protection.	transcription
67409	2	336056	7	NULL	NULL	0	NULL	NOE	Chemical		is a type of					ceramidase inhibitor	Chemical				NULL		0	NULL	NULL	NULL	gw70_neuropharmacology_45_8_1130_s_300	14614956	We assessed the effects of the ceramidase  inhibitor NOE and the sphingosine kinase inhibitor DMS ( [  Edsall et al., 1998]) on ceramide-induced neuro-protection.	transcription
67410	3	336056	7	NULL	NULL	0	NULL	DMS	Chemical		is a type of					sphingosine kinase inhibitor	Chemical				NULL		0	NULL	NULL	NULL	gw70_neuropharmacology_45_8_1130_s_300	14614956	We assessed the effects of the ceramidase  inhibitor NOE and the sphingosine kinase inhibitor DMS ( [  Edsall et al., 1998]) on ceramide-induced neuro-protection.	transcription
60691	1	336057	5	NULL	NULL	0	NULL	fumonisin B1	Chemical		block					ceramide	Chemical	production of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34290_s_6	15180992	Although fumonisin B1 blocked ceramide production and increased sphingosine, it did not reverse the negative effect of SPP-1 expression on EGF- or S1P-induced chemotaxis.	transcription
60692	2	336057	5	NULL	NULL	0	NULL	fumonisin B1	Chemical		increases					sphingosine	Chemical	production of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34290_s_6	15180992	Although fumonisin B1 blocked ceramide production and increased sphingosine, it did not reverse the negative effect of SPP-1 expression on EGF- or S1P-induced chemotaxis.	transcription
60693	3	336057	5	NULL	NULL	0	NULL	S1P	Chemical		induce					chemotaxis	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34290_s_6	15180992	Although fumonisin B1 blocked ceramide production and increased sphingosine, it did not reverse the negative effect of SPP-1 expression on EGF- or S1P-induced chemotaxis.	transcription
60694	4	336057	5	NULL	NULL	0	NULL	EGF	GP		induce					chemotaxis	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34290_s_6	15180992	Although fumonisin B1 blocked ceramide production and increased sphingosine, it did not reverse the negative effect of SPP-1 expression on EGF- or S1P-induced chemotaxis.	transcription
60695	5	336057	5	NULL	NULL	0	NULL	SPP-1	Chemical	expression of	effects		negatively			statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34290_s_6	15180992	Although fumonisin B1 blocked ceramide production and increased sphingosine, it did not reverse the negative effect of SPP-1 expression on EGF- or S1P-induced chemotaxis.	transcription
60696	6	336057	5	NULL	NULL	0	NULL	SPP-1	Chemical	expression of	effects		negatively			statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34290_s_6	15180992	Although fumonisin B1 blocked ceramide production and increased sphingosine, it did not reverse the negative effect of SPP-1 expression on EGF- or S1P-induced chemotaxis.	transcription
60697	7	336057	5	NULL	NULL	0	NULL	fumonisin B1	Chemical		does not reverse					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34290_s_6	15180992	Although fumonisin B1 blocked ceramide production and increased sphingosine, it did not reverse the negative effect of SPP-1 expression on EGF- or S1P-induced chemotaxis.	transcription
60698	8	336057	5	NULL	NULL	0	NULL	fumonisin B1	Chemical		does not reverse					statement 6	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34290_s_6	15180992	Although fumonisin B1 blocked ceramide production and increased sphingosine, it did not reverse the negative effect of SPP-1 expression on EGF- or S1P-induced chemotaxis.	transcription
67411	1	336057	7	NULL	NULL	0	NULL	fumonisin B1	Chemical		blocks					ceramide	Chemical	production of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34290_s_6	15180992	Although fumonisin B1 blocked ceramide production and increased sphingosine, it did not reverse the negative effect of SPP-1 expression on EGF- or S1P-induced chemotaxis.	transcription
67412	2	336057	7	NULL	NULL	0	NULL	fumonisin B1	Chemical		increase					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34290_s_6	15180992	Although fumonisin B1 blocked ceramide production and increased sphingosine, it did not reverse the negative effect of SPP-1 expression on EGF- or S1P-induced chemotaxis.	transcription
67413	3	336057	7	NULL	NULL	0	NULL	SPP-1	GP	expression of	effect		negatively			EGF	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34290_s_6	15180992	Although fumonisin B1 blocked ceramide production and increased sphingosine, it did not reverse the negative effect of SPP-1 expression on EGF- or S1P-induced chemotaxis.	transcription
67414	4	336057	7	NULL	NULL	0	NULL	S1P	Chemical		induce					chemotaxis	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34290_s_6	15180992	Although fumonisin B1 blocked ceramide production and increased sphingosine, it did not reverse the negative effect of SPP-1 expression on EGF- or S1P-induced chemotaxis.	transcription
67415	5	336057	7	NULL	NULL	0	NULL	SPP-1	GP	expression of	effect		negatively			statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34290_s_6	15180992	Although fumonisin B1 blocked ceramide production and increased sphingosine, it did not reverse the negative effect of SPP-1 expression on EGF- or S1P-induced chemotaxis.	transcription
67416	6	336057	7	NULL	NULL	0	NULL	fumonisin B1	Chemical		does not reverse					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34290_s_6	15180992	Although fumonisin B1 blocked ceramide production and increased sphingosine, it did not reverse the negative effect of SPP-1 expression on EGF- or S1P-induced chemotaxis.	transcription
67417	7	336057	7	NULL	NULL	0	NULL	fumonisin B1	Chemical		does not reverse					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34290_s_6	15180992	Although fumonisin B1 blocked ceramide production and increased sphingosine, it did not reverse the negative effect of SPP-1 expression on EGF- or S1P-induced chemotaxis.	transcription
67418	8	336057	7	NULL	NULL	0	NULL	statement 6	Process		is an alternative to					statement 7	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_33_34290_s_6	15180992	Although fumonisin B1 blocked ceramide production and increased sphingosine, it did not reverse the negative effect of SPP-1 expression on EGF- or S1P-induced chemotaxis.	transcription
60699	1	336058	5	NULL	NULL	0	NULL	L-Cycloserine	Chemical		inhibits					serine palmitoyltransferase	GP	activity of			NULL	in vitro and in vivo	0	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_51	12424251	L-Cycloserine and beta-chloro-L-alanine block sphingosine and ceramide biosynthesis by inhibiting serine palmitoyltransferase activity both  in vitro and  in vivo ( ,  ).	transcription
60700	2	336058	5	NULL	NULL	0	NULL	statement 1	Process		blocks					sphingosine	Chemical	biosynthesis of			NULL	in vitro and in vivo	0	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_51	12424251	L-Cycloserine and beta-chloro-L-alanine block sphingosine and ceramide biosynthesis by inhibiting serine palmitoyltransferase activity both  in vitro and  in vivo ( ,  ).	transcription
60701	3	336058	5	NULL	NULL	0	NULL	statement 1	Process		blocks					ceramide	Chemical	biosynthesis of			NULL	in vitro and in vivo	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_51	12424251	L-Cycloserine and beta-chloro-L-alanine block sphingosine and ceramide biosynthesis by inhibiting serine palmitoyltransferase activity both  in vitro and  in vivo ( ,  ).	transcription
60702	4	336058	5	NULL	NULL	0	NULL	beta-chloro-L-alanine	Chemical		inhibits					serine palmitoyltransferase	GP	activity of			NULL	in vitro and in vivo	0	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_51	12424251	L-Cycloserine and beta-chloro-L-alanine block sphingosine and ceramide biosynthesis by inhibiting serine palmitoyltransferase activity both  in vitro and  in vivo ( ,  ).	transcription
60703	5	336058	5	NULL	NULL	0	NULL	statement 4	Process		blocks					sphingosine	Chemical	biosynthesis of			NULL	in vitro and in vivo	0	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_51	12424251	L-Cycloserine and beta-chloro-L-alanine block sphingosine and ceramide biosynthesis by inhibiting serine palmitoyltransferase activity both  in vitro and  in vivo ( ,  ).	transcription
60704	6	336058	5	NULL	NULL	0	NULL	statement 4	Process		blocks					ceramide	Chemical	biosynthesis of			NULL	in vitro and in vivo	0	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_51	12424251	L-Cycloserine and beta-chloro-L-alanine block sphingosine and ceramide biosynthesis by inhibiting serine palmitoyltransferase activity both  in vitro and  in vivo ( ,  ).	transcription
67419	1	336058	7	NULL	NULL	0	NULL	L-Cycloserine	AminoAcid		block					sphingosine	Chemical	biosynthesis of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_51	12424251	L-Cycloserine and beta-chloro-L-alanine block sphingosine and ceramide biosynthesis by inhibiting serine palmitoyltransferase activity both  in vitro and  in vivo ( ,  ).	transcription
67420	2	336058	7	NULL	NULL	NULL	NULL	 beta-chloro-L-alanine	AminoAcid		block					sphingosine	Chemical	biosynthesis of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_51	12424251	L-Cycloserine and beta-chloro-L-alanine block sphingosine and ceramide biosynthesis by inhibiting serine palmitoyltransferase activity both  in vitro and  in vivo ( ,  ).	transcription
67421	3	336058	7	NULL	NULL	0	NULL	L-Cycloserine	AminoAcid		block					ceramide	Chemical	biosynthesis of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_51	12424251	L-Cycloserine and beta-chloro-L-alanine block sphingosine and ceramide biosynthesis by inhibiting serine palmitoyltransferase activity both  in vitro and  in vivo ( ,  ).	transcription
67424	4	336058	7	NULL	NULL	0	NULL	beta-chloro-L-alanine	Chemical		block					ceramide	Chemical	biosynthesis of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_51	12424251	L-Cycloserine and beta-chloro-L-alanine block sphingosine and ceramide biosynthesis by inhibiting serine palmitoyltransferase activity both  in vitro and  in vivo ( ,  ).	transcription
67439	5	336058	7	NULL	NULL	0	NULL	statement 1	Process		occur by					serine palmitoyltransferase activity	Process	inhibition of			NULL	in vitro	0	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_51	12424251	L-Cycloserine and beta-chloro-L-alanine block sphingosine and ceramide biosynthesis by inhibiting serine palmitoyltransferase activity both  in vitro and  in vivo ( ,  ).	transcription
67440	6	336058	7	NULL	NULL	NULL	NULL	statement 1	Process		occur by					serine palmitoyltransferase activity	Process	inhibition of			NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_51	12424251	L-Cycloserine and beta-chloro-L-alanine block sphingosine and ceramide biosynthesis by inhibiting serine palmitoyltransferase activity both  in vitro and  in vivo ( ,  ).	transcription
67441	7	336058	7	NULL	NULL	NULL	NULL	statement 2	Process		occur by					serine palmitoyltransferase activity	Process	inhibition of			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_51	12424251	L-Cycloserine and beta-chloro-L-alanine block sphingosine and ceramide biosynthesis by inhibiting serine palmitoyltransferase activity both  in vitro and  in vivo ( ,  ).	transcription
67442	8	336058	7	NULL	NULL	0	NULL	statement 2	Process		occur by					serine palmitoyltransferase activity	Process	inhibition of			NULL	in vivo	0	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_51	12424251	L-Cycloserine and beta-chloro-L-alanine block sphingosine and ceramide biosynthesis by inhibiting serine palmitoyltransferase activity both  in vitro and  in vivo ( ,  ).	transcription
67443	9	336058	7	NULL	NULL	NULL	NULL	statement 3	Process		occur by					serine palmitoyltransferase activity	Process	inhibition of			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_51	12424251	L-Cycloserine and beta-chloro-L-alanine block sphingosine and ceramide biosynthesis by inhibiting serine palmitoyltransferase activity both  in vitro and  in vivo ( ,  ).	transcription
67444	10	336058	7	NULL	NULL	NULL	NULL	statement 3	Process		occur by					serine palmitoyltransferase activity	Process	inhibition of			NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_51	12424251	L-Cycloserine and beta-chloro-L-alanine block sphingosine and ceramide biosynthesis by inhibiting serine palmitoyltransferase activity both  in vitro and  in vivo ( ,  ).	transcription
67445	11	336058	7	NULL	NULL	0	NULL	statement 4	Process		occur by					serine palmitoyltransferase activity	Process	inhibition of			NULL	in vitro	0	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_51	12424251	L-Cycloserine and beta-chloro-L-alanine block sphingosine and ceramide biosynthesis by inhibiting serine palmitoyltransferase activity both  in vitro and  in vivo ( ,  ).	transcription
67446	12	336058	7	NULL	NULL	NULL	NULL	statement 4	Process		occur by					serine palmitoyltransferase activity	Process	inhibition of			NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_2_974_s_51	12424251	L-Cycloserine and beta-chloro-L-alanine block sphingosine and ceramide biosynthesis by inhibiting serine palmitoyltransferase activity both  in vitro and  in vivo ( ,  ).	transcription
60705	1	336059	5	NULL	NULL	0	NULL	sphingosine	Chemical		is phosphorylated to					S1P	Chemical				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_8_s_52	12069805	S1P, produced by phosphorylation of sphingosine by SPHK ( Fig. 1 and  Fig. 2), suppresses ceramide-induced apoptosis and stimulates mitogenic pathways [ 1,  2,  3 and  6].	transcription
60706	2	336059	5	NULL	NULL	0	NULL	SPHK	GP		catalyzes					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_8_s_52	12069805	S1P, produced by phosphorylation of sphingosine by SPHK ( Fig. 1 and  Fig. 2), suppresses ceramide-induced apoptosis and stimulates mitogenic pathways [ 1,  2,  3 and  6].	transcription
60707	3	336059	5	NULL	NULL	0	NULL	apoptosis	Process		is induced by					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_8_s_52	12069805	S1P, produced by phosphorylation of sphingosine by SPHK ( Fig. 1 and  Fig. 2), suppresses ceramide-induced apoptosis and stimulates mitogenic pathways [ 1,  2,  3 and  6].	transcription
60708	4	336059	5	NULL	NULL	0	NULL	S1P	Chemical		suppress					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_8_s_52	12069805	S1P, produced by phosphorylation of sphingosine by SPHK ( Fig. 1 and  Fig. 2), suppresses ceramide-induced apoptosis and stimulates mitogenic pathways [ 1,  2,  3 and  6].	transcription
60709	5	336059	5	NULL	NULL	0	NULL	S1P	Chemical		stimulates					mitogenic pathways	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_8_s_52	12069805	S1P, produced by phosphorylation of sphingosine by SPHK ( Fig. 1 and  Fig. 2), suppresses ceramide-induced apoptosis and stimulates mitogenic pathways [ 1,  2,  3 and  6].	transcription
67425	1	336059	7	NULL	NULL	0	NULL	S1P	Chemical		produced by					sphingosine	Chemical	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_8_s_52	12069805	S1P, produced by phosphorylation of sphingosine by SPHK ( Fig. 1 and  Fig. 2), suppresses ceramide-induced apoptosis and stimulates mitogenic pathways [ 1,  2,  3 and  6].	transcription
67426	2	336059	7	NULL	NULL	0	NULL	SPHK			catalyze					statement 1					NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_8_s_52	12069805	S1P, produced by phosphorylation of sphingosine by SPHK ( Fig. 1 and  Fig. 2), suppresses ceramide-induced apoptosis and stimulates mitogenic pathways [ 1,  2,  3 and  6].	transcription
67427	3	336059	7	NULL	NULL	0	NULL	ceramide	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_8_s_52	12069805	S1P, produced by phosphorylation of sphingosine by SPHK ( Fig. 1 and  Fig. 2), suppresses ceramide-induced apoptosis and stimulates mitogenic pathways [ 1,  2,  3 and  6].	transcription
67428	4	336059	7	NULL	NULL	0	NULL	S1P	Chemical		suppress					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_8_s_52	12069805	S1P, produced by phosphorylation of sphingosine by SPHK ( Fig. 1 and  Fig. 2), suppresses ceramide-induced apoptosis and stimulates mitogenic pathways [ 1,  2,  3 and  6].	transcription
67429	5	336059	7	NULL	NULL	0	NULL	S1P	Chemical		stimulates					mitogenic pathways	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_8_s_52	12069805	S1P, produced by phosphorylation of sphingosine by SPHK ( Fig. 1 and  Fig. 2), suppresses ceramide-induced apoptosis and stimulates mitogenic pathways [ 1,  2,  3 and  6].	transcription
60710	1	336060	5	NULL	NULL	0	NULL	sphingosine 1-phosphate	Chemical		inhibits					caspases	GP	activation of			NULL	Jurkat T lymphocytes	0	NULL	NULL	NULL	gw60_currbiol_10_23_1527_s_121	11114522	Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide- mediated apoptosis in Jurkat T lymphocytes.	transcription
60711	2	336060	5	NULL	NULL	0	NULL	caspases	GP		cleave					poly(ADP-ribose) polymerase	GP				NULL	Jurkat T lymphocytes	0	NULL	NULL	NULL	gw60_currbiol_10_23_1527_s_121	11114522	Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide- mediated apoptosis in Jurkat T lymphocytes.	transcription
60712	3	336060	5	NULL	NULL	0	NULL	caspases	GP		cleave					lamins	GP				NULL	Jurkat T lymphocytes	0	NULL	NULL	NULL	gw60_currbiol_10_23_1527_s_121	11114522	Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide- mediated apoptosis in Jurkat T lymphocytes.	transcription
60713	4	336060	5	NULL	NULL	0	NULL	apoptosis	Process		is mediated by					Fas	GP				NULL	Jurkat T lymphocytes	NULL	NULL	NULL	NULL	gw60_currbiol_10_23_1527_s_121	11114522	Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide- mediated apoptosis in Jurkat T lymphocytes.	transcription
60714	5	336060	5	NULL	NULL	0	NULL	apoptosis	Process		is mediated by					ceramide	Chemical				NULL	Jurkat T lymphocytes	0	NULL	NULL	NULL	gw60_currbiol_10_23_1527_s_121	11114522	Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide- mediated apoptosis in Jurkat T lymphocytes.	transcription
60715	6	336060	5	NULL	NULL	0	NULL	statement 2	Process		occurs during					statement 4	Process				NULL	Jurkat T lymphocytes	0	NULL	NULL	NULL	gw60_currbiol_10_23_1527_s_121	11114522	Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide- mediated apoptosis in Jurkat T lymphocytes.	transcription
60716	7	336060	5	NULL	NULL	0	NULL	statement 2	Process		occurs during					statement 5	Process				NULL	Jurkat T lymphocytes	0	NULL	NULL	NULL	gw60_currbiol_10_23_1527_s_121	11114522	Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide- mediated apoptosis in Jurkat T lymphocytes.	transcription
60717	8	336060	5	NULL	NULL	0	NULL	statement 3	Process		occurs during					statement 4	Process				NULL	Jurkat T lymphocytes	NULL	NULL	NULL	NULL	gw60_currbiol_10_23_1527_s_121	11114522	Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide- mediated apoptosis in Jurkat T lymphocytes.	transcription
60718	9	336060	5	NULL	NULL	0	NULL	statement 3	Process		occurs during					statement 5	Process				NULL	Jurkat T lymphocytes	0	NULL	NULL	NULL	gw60_currbiol_10_23_1527_s_121	11114522	Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide- mediated apoptosis in Jurkat T lymphocytes.	transcription
67430	1	336060	7	NULL	NULL	0	NULL	Sphingosine 1-phosphate	Chemical		inhibits					caspases	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_currbiol_10_23_1527_s_121	11114522	Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide- mediated apoptosis in Jurkat T lymphocytes.	transcription
67431	2	336060	7	NULL	NULL	NULL	NULL	caspases	GP		cleave					poly(ADP-ribose) polymerase	GP				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_23_1527_s_121	11114522	Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide- mediated apoptosis in Jurkat T lymphocytes.	transcription
67432	3	336060	7	NULL	NULL	0	NULL	caspases	GP		cleave					lamins	GP				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_23_1527_s_121	11114522	Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide- mediated apoptosis in Jurkat T lymphocytes.	transcription
67433	4	336060	7	NULL	NULL	NULL	NULL	Fas	GP		mediates					apoptosis 	Process				NULL	Jurkat T lymphocytes	NULL	NULL	NULL	NULL	gw60_currbiol_10_23_1527_s_121	11114522	Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide- mediated apoptosis in Jurkat T lymphocytes.	transcription
67434	5	336060	7	NULL	NULL	0	NULL	ceramide	Chemical		mediates					apoptosis	Process				NULL	Jurkat T lymphocytes	0	NULL	NULL	NULL	gw60_currbiol_10_23_1527_s_121	11114522	Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide- mediated apoptosis in Jurkat T lymphocytes.	transcription
67435	6	336060	7	NULL	NULL	NULL	NULL	statement 2	Process		occur during					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_currbiol_10_23_1527_s_121	11114522	Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide- mediated apoptosis in Jurkat T lymphocytes.	transcription
67436	7	336060	7	NULL	NULL	0	NULL	statement 2	Process		occur during					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_23_1527_s_121	11114522	Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide- mediated apoptosis in Jurkat T lymphocytes.	transcription
67437	8	336060	7	NULL	NULL	0	NULL	statement 3	Process		occur during					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_23_1527_s_121	11114522	Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide- mediated apoptosis in Jurkat T lymphocytes.	transcription
67438	9	336060	7	NULL	NULL	0	NULL	statement 3	Process		occur during					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_currbiol_10_23_1527_s_121	11114522	Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide- mediated apoptosis in Jurkat T lymphocytes.	transcription
60719	1	336061	5	NULL	NULL	0	NULL	C2-ceramide	Chemical	treatment;;exogenous	increases					ceramide	Chemical	endogenous			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_23_1_163_s_26	12482970	It was further shown that treatment of cells with exogenous C2-ceramide not only increases the level of endogenous ceramide but also leads to a marked increase in the level of cellular sphingosine ( 9).	transcription
60720	2	336061	5	NULL	NULL	0	NULL	C2-ceramide	Chemical	treatment;;exogenous	increases					sphingosine	Chemical	cellular levels of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_1_163_s_26	12482970	It was further shown that treatment of cells with exogenous C2-ceramide not only increases the level of endogenous ceramide but also leads to a marked increase in the level of cellular sphingosine ( 9).	transcription
67447	1	336061	7	NULL	NULL	0	NULL	C2-ceramide	Chemical	exogenous	increase					ceramide	Chemical	level of endogenous			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_1_163_s_26	12482970	It was further shown that treatment of cells with exogenous C2-ceramide not only increases the level of endogenous ceramide but also leads to a marked increase in the level of cellular sphingosine ( 9).	transcription
67448	2	336061	7	NULL	NULL	0	NULL	C2-ceramide	Chemical	exogenous	increase					cellular sphingosine	Chemical	levels of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_1_163_s_26	12482970	It was further shown that treatment of cells with exogenous C2-ceramide not only increases the level of endogenous ceramide but also leads to a marked increase in the level of cellular sphingosine ( 9).	transcription
60721	1	336063	5	NULL	NULL	0	NULL	CERK	GP		is homologous to					SPK	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23294_s_263	11956206	Although CERK is somewhat homologous to SPK, especially in the previously identified conserved domains ( 28), it is highly specific for ceramide as substrate and does not catalyze phosphorylation of sphingosine or diacylglycerol.	transcription
60722	2	336063	5	NULL	NULL	0	NULL	CERK	GP		is specific for		highly			ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23294_s_263	11956206	Although CERK is somewhat homologous to SPK, especially in the previously identified conserved domains ( 28), it is highly specific for ceramide as substrate and does not catalyze phosphorylation of sphingosine or diacylglycerol.	transcription
60723	3	336063	5	NULL	NULL	0	NULL	CERK	GP		does not catalyze					sphingosine	Chemical	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23294_s_263	11956206	Although CERK is somewhat homologous to SPK, especially in the previously identified conserved domains ( 28), it is highly specific for ceramide as substrate and does not catalyze phosphorylation of sphingosine or diacylglycerol.	transcription
60724	4	336063	5	NULL	NULL	0	NULL	CERK	GP		does not catalyze					diacylglycerol	Chemical	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23294_s_263	11956206	Although CERK is somewhat homologous to SPK, especially in the previously identified conserved domains ( 28), it is highly specific for ceramide as substrate and does not catalyze phosphorylation of sphingosine or diacylglycerol.	transcription
60725	5	336063	5	NULL	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23294_s_263	11956206	Although CERK is somewhat homologous to SPK, especially in the previously identified conserved domains ( 28), it is highly specific for ceramide as substrate and does not catalyze phosphorylation of sphingosine or diacylglycerol.	transcription
67449	1	336063	7	NULL	NULL	0	NULL	CERK	GP		homologous to					SPK	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23294_s_263	11956206	Although CERK is somewhat homologous to SPK, especially in the previously identified conserved domains ( 28), it is highly specific for ceramide as substrate and does not catalyze phosphorylation of sphingosine or diacylglycerol.	transcription
67450	2	336063	7	NULL	NULL	0	NULL	ceramide	Chemical		substrate for					CERK	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23294_s_263	11956206	Although CERK is somewhat homologous to SPK, especially in the previously identified conserved domains ( 28), it is highly specific for ceramide as substrate and does not catalyze phosphorylation of sphingosine or diacylglycerol.	transcription
67451	3	336063	7	NULL	NULL	0	NULL	CERK	GP		does not catalyze					sphingosine	Chemical	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23294_s_263	11956206	Although CERK is somewhat homologous to SPK, especially in the previously identified conserved domains ( 28), it is highly specific for ceramide as substrate and does not catalyze phosphorylation of sphingosine or diacylglycerol.	transcription
67452	4	336063	7	NULL	NULL	0	NULL	CERK	GP		does not catalyze					diacylglycerol	Chemical	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23294_s_263	11956206	Although CERK is somewhat homologous to SPK, especially in the previously identified conserved domains ( 28), it is highly specific for ceramide as substrate and does not catalyze phosphorylation of sphingosine or diacylglycerol.	transcription
60726	1	336064	5	NULL	NULL	0	NULL	ceramide	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_193	10747891	Because ceramide and sphingosine induce apoptosis in a Bcl-xL-dependent manner, we determined whether they were also capable of mediating caspase-8 activation.	transcription
60727	2	336064	5	NULL	NULL	0	NULL	statement 1	Process		is dependent on					Bcl-xL	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_193	10747891	Because ceramide and sphingosine induce apoptosis in a Bcl-xL-dependent manner, we determined whether they were also capable of mediating caspase-8 activation.	transcription
60728	3	336064	5	NULL	NULL	0	NULL	sphingosine	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_193	10747891	Because ceramide and sphingosine induce apoptosis in a Bcl-xL-dependent manner, we determined whether they were also capable of mediating caspase-8 activation.	transcription
60729	4	336064	5	NULL	NULL	0	NULL	statement 3	Process		is dependent on					Bcl-xL	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_193	10747891	Because ceramide and sphingosine induce apoptosis in a Bcl-xL-dependent manner, we determined whether they were also capable of mediating caspase-8 activation.	transcription
67453	1	336064	7	NULL	NULL	0	NULL	ceramide	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_193	10747891	Because ceramide and sphingosine induce apoptosis in a Bcl-xL-dependent manner, we determined whether they were also capable of mediating caspase-8 activation.	transcription
67454	2	336064	7	NULL	NULL	0	NULL	sphingosine	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_193	10747891	Because ceramide and sphingosine induce apoptosis in a Bcl-xL-dependent manner, we determined whether they were also capable of mediating caspase-8 activation.	transcription
67455	3	336064	7	NULL	NULL	0	NULL	statement 1	Process		depends on					Bcl-xL	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_193	10747891	Because ceramide and sphingosine induce apoptosis in a Bcl-xL-dependent manner, we determined whether they were also capable of mediating caspase-8 activation.	transcription
67456	4	336064	7	NULL	NULL	0	NULL	statement 2	Process		depends on					Bcl-xL	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_193	10747891	Because ceramide and sphingosine induce apoptosis in a Bcl-xL-dependent manner, we determined whether they were also capable of mediating caspase-8 activation.	transcription
60730	1	336065	5	NULL	NULL	0	NULL	ceramide	Chemical	apoptotic response to	is regulated by		indirectly			sphingosine & diglyceride	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_38	8626522	Thus, it  appears that the apoptotic response to ceramide is indirectly regulated  by the combined actions of sphingosine and diglyceride, which  respectively limit or extend the cytoprotective influence of PKC.	transcription
60731	2	336065	5	NULL	NULL	0	NULL	statement 1	Process		limits					PKC	GP	cytoprotective influence of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_38	8626522	Thus, it  appears that the apoptotic response to ceramide is indirectly regulated  by the combined actions of sphingosine and diglyceride, which  respectively limit or extend the cytoprotective influence of PKC.	transcription
60732	3	336065	5	NULL	NULL	0	NULL	statement 1	Process		extends					PKC	GP	cytoprotective influence of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_38	8626522	Thus, it  appears that the apoptotic response to ceramide is indirectly regulated  by the combined actions of sphingosine and diglyceride, which  respectively limit or extend the cytoprotective influence of PKC.	transcription
60733	4	336065	5	NULL	NULL	0	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_38	8626522	Thus, it  appears that the apoptotic response to ceramide is indirectly regulated  by the combined actions of sphingosine and diglyceride, which  respectively limit or extend the cytoprotective influence of PKC.	transcription
67457	1	336065	7	NULL	NULL	0	NULL	ceramide	Chemical		shows					apoptotic response	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_38	8626522	Thus, it  appears that the apoptotic response to ceramide is indirectly regulated  by the combined actions of sphingosine and diglyceride, which  respectively limit or extend the cytoprotective influence of PKC.	transcription
67458	2	336065	7	NULL	NULL	NULL	NULL	statement 1	Process		 regulated by		indirectly			sphingosine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_38	8626522	Thus, it  appears that the apoptotic response to ceramide is indirectly regulated  by the combined actions of sphingosine and diglyceride, which  respectively limit or extend the cytoprotective influence of PKC.	transcription
67459	3	336065	7	NULL	NULL	0	NULL	statement 1	Process		regulated by		indirectly			diglyceride	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_38	8626522	Thus, it  appears that the apoptotic response to ceramide is indirectly regulated  by the combined actions of sphingosine and diglyceride, which  respectively limit or extend the cytoprotective influence of PKC.	transcription
67460	4	336065	7	NULL	NULL	NULL	NULL	statement 2	Process		limit					PKC	GP	cytoprotective influence of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_38	8626522	Thus, it  appears that the apoptotic response to ceramide is indirectly regulated  by the combined actions of sphingosine and diglyceride, which  respectively limit or extend the cytoprotective influence of PKC.	transcription
67461	5	336065	7	NULL	NULL	0	NULL	statement 3	Process		extend					PKC	GP	cytoprotective influence of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_38	8626522	Thus, it  appears that the apoptotic response to ceramide is indirectly regulated  by the combined actions of sphingosine and diglyceride, which  respectively limit or extend the cytoprotective influence of PKC.	transcription
60734	1	336066	5	NULL	NULL	0	NULL	cell death	Process		is dependent on					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_263	8626522	First, as  already noted, sphingosine and sphinganine exhibited equivalent potency  and efficacy in both the direct induction of apoptosis and the  potentiation of ceramide-dependent cell death.	transcription
60735	2	336066	5	NULL	NULL	0	NULL	sphingosine	Chemical		induce		directly			apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_263	8626522	First, as  already noted, sphingosine and sphinganine exhibited equivalent potency  and efficacy in both the direct induction of apoptosis and the  potentiation of ceramide-dependent cell death.	transcription
60736	3	336066	5	NULL	NULL	0	NULL	sphinganine	Chemical		induce		directly			apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_263	8626522	First, as  already noted, sphingosine and sphinganine exhibited equivalent potency  and efficacy in both the direct induction of apoptosis and the  potentiation of ceramide-dependent cell death.	transcription
60737	4	336066	5	NULL	NULL	0	NULL	sphingosine	Chemical		potentiate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_263	8626522	First, as  already noted, sphingosine and sphinganine exhibited equivalent potency  and efficacy in both the direct induction of apoptosis and the  potentiation of ceramide-dependent cell death.	transcription
60738	5	336066	5	NULL	NULL	0	NULL	sphinganine	Chemical		potentiate					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_263	8626522	First, as  already noted, sphingosine and sphinganine exhibited equivalent potency  and efficacy in both the direct induction of apoptosis and the  potentiation of ceramide-dependent cell death.	transcription
60739	6	336066	5	NULL	NULL	0	NULL	statement 2	Process	potency of	is equivalent to					statement 3	Process	potency of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_263	8626522	First, as  already noted, sphingosine and sphinganine exhibited equivalent potency  and efficacy in both the direct induction of apoptosis and the  potentiation of ceramide-dependent cell death.	transcription
60740	7	336066	5	NULL	NULL	0	NULL	statement 2	Process	efficacy of	is equivalent to					statement 3	Process	efficacy of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_263	8626522	First, as  already noted, sphingosine and sphinganine exhibited equivalent potency  and efficacy in both the direct induction of apoptosis and the  potentiation of ceramide-dependent cell death.	transcription
60741	8	336066	5	NULL	NULL	0	NULL	statement 4	Process	potency of	is equivalent to					statement 5	Process	potency of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_263	8626522	First, as  already noted, sphingosine and sphinganine exhibited equivalent potency  and efficacy in both the direct induction of apoptosis and the  potentiation of ceramide-dependent cell death.	transcription
60742	9	336066	5	NULL	NULL	0	NULL	statement 4	Process	efficacy of	is equivalent to					statement 5	Process	efficacy of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_263	8626522	First, as  already noted, sphingosine and sphinganine exhibited equivalent potency  and efficacy in both the direct induction of apoptosis and the  potentiation of ceramide-dependent cell death.	transcription
67462	1	336066	7	NULL	NULL	0	NULL	sphingosine	Chemical		induce		directly			apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_263	8626522	First, as  already noted, sphingosine and sphinganine exhibited equivalent potency  and efficacy in both the direct induction of apoptosis and the  potentiation of ceramide-dependent cell death.	transcription
67463	2	336066	7	NULL	NULL	NULL	NULL	sphinganine	Chemical		induce		directly			apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_263	8626522	First, as  already noted, sphingosine and sphinganine exhibited equivalent potency  and efficacy in both the direct induction of apoptosis and the  potentiation of ceramide-dependent cell death.	transcription
67464	3	336066	7	NULL	NULL	0	NULL	cell death	Process		depends on					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_263	8626522	First, as  already noted, sphingosine and sphinganine exhibited equivalent potency  and efficacy in both the direct induction of apoptosis and the  potentiation of ceramide-dependent cell death.	transcription
67465	4	336066	7	NULL	NULL	0	NULL	sphingosine	Chemical		potentiate					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_263	8626522	First, as  already noted, sphingosine and sphinganine exhibited equivalent potency  and efficacy in both the direct induction of apoptosis and the  potentiation of ceramide-dependent cell death.	transcription
67466	5	336066	7	NULL	NULL	0	NULL	sphinganine	Chemical		potentiate					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_263	8626522	First, as  already noted, sphingosine and sphinganine exhibited equivalent potency  and efficacy in both the direct induction of apoptosis and the  potentiation of ceramide-dependent cell death.	transcription
60743	1	336067	5	NULL	NULL	0	NULL	ceramide	Chemical		deacetylated to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_28_16506_s_25	8663293	Deacylation of ceramide produces sphingosine which inhibits protein kinase C ( 20) and Mg2+-dependent and -independent PAP activities ( 24,  25).	transcription
60744	2	336067	5	NULL	NULL	0	NULL	sphingosine	Chemical		inhibits					protein kinase C	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_28_16506_s_25	8663293	Deacylation of ceramide produces sphingosine which inhibits protein kinase C ( 20) and Mg2+-dependent and -independent PAP activities ( 24,  25).	transcription
60745	3	336067	5	NULL	NULL	0	NULL	PAP	GP	activity of	is dependent on					Mg2+	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_28_16506_s_25	8663293	Deacylation of ceramide produces sphingosine which inhibits protein kinase C ( 20) and Mg2+-dependent and -independent PAP activities ( 24,  25).	transcription
60746	4	336067	5	NULL	NULL	0	NULL	PAP	GP	activity of	is independent of					Mg2+	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_28_16506_s_25	8663293	Deacylation of ceramide produces sphingosine which inhibits protein kinase C ( 20) and Mg2+-dependent and -independent PAP activities ( 24,  25).	transcription
60747	5	336067	5	NULL	NULL	0	NULL	sphingosine	Chemical		inhibits					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_28_16506_s_25	8663293	Deacylation of ceramide produces sphingosine which inhibits protein kinase C ( 20) and Mg2+-dependent and -independent PAP activities ( 24,  25).	transcription
60748	6	336067	5	NULL	NULL	0	NULL	sphingosine	Chemical		inhibits					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_28_16506_s_25	8663293	Deacylation of ceramide produces sphingosine which inhibits protein kinase C ( 20) and Mg2+-dependent and -independent PAP activities ( 24,  25).	transcription
67467	1	336067	7	NULL	NULL	0	NULL	ceramide	Chemical	deacylation of	produce					sphingosine 	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_28_16506_s_25	8663293	Deacylation of ceramide produces sphingosine which inhibits protein kinase C ( 20) and Mg2+-dependent and -independent PAP activities ( 24,  25).	transcription
67468	2	336067	7	NULL	NULL	0	NULL	sphingosine	Chemical		inhibit					protein kinase C	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_28_16506_s_25	8663293	Deacylation of ceramide produces sphingosine which inhibits protein kinase C ( 20) and Mg2+-dependent and -independent PAP activities ( 24,  25).	transcription
67469	3	336067	7	NULL	NULL	0	NULL	PAP activities	Process		depend on					Mg2+	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_28_16506_s_25	8663293	Deacylation of ceramide produces sphingosine which inhibits protein kinase C ( 20) and Mg2+-dependent and -independent PAP activities ( 24,  25).	transcription
67470	4	336067	7	NULL	NULL	0	NULL	PAP activities	Process		independent of					Mg2+ 	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_28_16506_s_25	8663293	Deacylation of ceramide produces sphingosine which inhibits protein kinase C ( 20) and Mg2+-dependent and -independent PAP activities ( 24,  25).	transcription
67471	5	336067	7	NULL	NULL	0	NULL	sphingosine	Chemical		inhibit					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_28_16506_s_25	8663293	Deacylation of ceramide produces sphingosine which inhibits protein kinase C ( 20) and Mg2+-dependent and -independent PAP activities ( 24,  25).	transcription
67472	6	336067	7	NULL	NULL	0	NULL	sphingosine	Chemical		inhibit					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_28_16506_s_25	8663293	Deacylation of ceramide produces sphingosine which inhibits protein kinase C ( 20) and Mg2+-dependent and -independent PAP activities ( 24,  25).	transcription
60749	1	336068	5	NULL	NULL	0	NULL	DL- threo-dihydrosphingosine	Chemical		increases					c-jun	GP	expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_45_27326_s_203	7592995	We found that DL- threo-dihydrosphingosine rather increased  c- jun  expression,   suggesting that sphingosine  1-phosphate is not involved in c- jun  induction by ceramide.	transcription
60750	2	336068	5	NULL	NULL	0	NULL	c- jun	Chemical		is induced by					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_45_27326_s_203	7592995	We found that DL- threo-dihydrosphingosine rather increased  c- jun  expression,   suggesting that sphingosine  1-phosphate is not involved in c- jun  induction by ceramide.	transcription
60751	3	336068	5	NULL	NULL	0	NULL	sphingosine 1-phosphate	Chemical		is not involved in					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_45_27326_s_203	7592995	We found that DL- threo-dihydrosphingosine rather increased  c- jun  expression,   suggesting that sphingosine  1-phosphate is not involved in c- jun  induction by ceramide.	transcription
60752	4	336068	5	NULL	NULL	0	NULL	statement 1	Process		suggest					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_45_27326_s_203	7592995	We found that DL- threo-dihydrosphingosine rather increased  c- jun  expression,   suggesting that sphingosine  1-phosphate is not involved in c- jun  induction by ceramide.	transcription
67473	1	336068	7	NULL	NULL	0	NULL	DL- threo-dihydrosphingosine	Chemical		increase					c-jun	GP	expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_45_27326_s_203	7592995	We found that DL- threo-dihydrosphingosine rather increased  c- jun  expression,   suggesting that sphingosine  1-phosphate is not involved in c- jun  induction by ceramide.	transcription
67474	2	336068	7	NULL	NULL	0	NULL	ceramide	Chemical		induce					c-jun	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_45_27326_s_203	7592995	We found that DL- threo-dihydrosphingosine rather increased  c- jun  expression,   suggesting that sphingosine  1-phosphate is not involved in c- jun  induction by ceramide.	transcription
67475	3	336068	7	NULL	NULL	0	NULL	sphingosine 1-phosphate	GP		is not involved in					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_45_27326_s_203	7592995	We found that DL- threo-dihydrosphingosine rather increased  c- jun  expression,   suggesting that sphingosine  1-phosphate is not involved in c- jun  induction by ceramide.	transcription
67476	4	336068	7	NULL	NULL	0	NULL	statement 1	Process		suggest					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_45_27326_s_203	7592995	We found that DL- threo-dihydrosphingosine rather increased  c- jun  expression,   suggesting that sphingosine  1-phosphate is not involved in c- jun  induction by ceramide.	transcription
60753	1	336069	5	NULL	NULL	0	NULL	SPP	Chemical		bind					Edg-3	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_8_4626_s_105	9988698	Sphingosine had a small but statistically significant effect on SPP binding to both Edg-3 and H218, while ceramide had a similarly small effect on binding to H218 only.	transcription
60754	2	336069	5	NULL	NULL	0	NULL	SPP	Chemical		bind					H218	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_8_4626_s_105	9988698	Sphingosine had a small but statistically significant effect on SPP binding to both Edg-3 and H218, while ceramide had a similarly small effect on binding to H218 only.	transcription
60755	3	336069	5	NULL	NULL	0	NULL	sphingosine	Chemical		effects		significantly			statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_8_4626_s_105	9988698	Sphingosine had a small but statistically significant effect on SPP binding to both Edg-3 and H218, while ceramide had a similarly small effect on binding to H218 only.	transcription
60756	4	336069	5	NULL	NULL	0	NULL	sphingosine	Chemical		effects		significantly			statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_8_4626_s_105	9988698	Sphingosine had a small but statistically significant effect on SPP binding to both Edg-3 and H218, while ceramide had a similarly small effect on binding to H218 only.	transcription
60757	5	336069	5	NULL	NULL	0	NULL	ceramide	Chemical		effects					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_8_4626_s_105	9988698	Sphingosine had a small but statistically significant effect on SPP binding to both Edg-3 and H218, while ceramide had a similarly small effect on binding to H218 only.	transcription
67477	1	336069	7	NULL	NULL	0	NULL	SPP	Chemical		bind					Edg-3	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_8_4626_s_105	9988698	Sphingosine had a small but statistically significant effect on SPP binding to both Edg-3 and H218, while ceramide had a similarly small effect on binding to H218 only.	transcription
67478	2	336069	7	NULL	NULL	NULL	NULL	SPP	Chemical		bind					H218	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_8_4626_s_105	9988698	Sphingosine had a small but statistically significant effect on SPP binding to both Edg-3 and H218, while ceramide had a similarly small effect on binding to H218 only.	transcription
67479	3	336069	7	NULL	NULL	0	NULL	Sphingosine	Chemical		effect		significantly			statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_8_4626_s_105	9988698	Sphingosine had a small but statistically significant effect on SPP binding to both Edg-3 and H218, while ceramide had a similarly small effect on binding to H218 only.	transcription
67480	4	336069	7	NULL	NULL	0	NULL	sphingosine	Chemical		effect		significantly			statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_8_4626_s_105	9988698	Sphingosine had a small but statistically significant effect on SPP binding to both Edg-3 and H218, while ceramide had a similarly small effect on binding to H218 only.	transcription
67481	5	336069	7	NULL	NULL	0	NULL	ceramide	Chemical		effect on		small			statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_8_4626_s_105	9988698	Sphingosine had a small but statistically significant effect on SPP binding to both Edg-3 and H218, while ceramide had a similarly small effect on binding to H218 only.	transcription
60765	1	336070	5	NULL	NULL	0	NULL	apoptosis	Process		is induced by					phorbol ester	Chemical				NULL	adherent HL-60 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_25_15345_s_25	9624115	The principal mediator of apoptosis in these cases is ceramide, not sphingosine, but SPP could be equally effective in the protection of adherent HL-60 cells from phorbol ester-induced apoptosis.	transcription
60768	2	336070	5	NULL	NULL	0	NULL	SPP	Chemical		protects					statement 1	Process				NULL	adherent HL-60 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_25_15345_s_25	9624115	The principal mediator of apoptosis in these cases is ceramide, not sphingosine, but SPP could be equally effective in the protection of adherent HL-60 cells from phorbol ester-induced apoptosis.	transcription
60787	3	336070	5	NULL	NULL	0	NULL	ceramide	Chemical		mediates					apoptosis	Process				NULL	adherent HL-60 cells	0	NULL	NULL	NULL	gw60_jbiolchem_273_25_15345_s_25	9624115	The principal mediator of apoptosis in these cases is ceramide, not sphingosine, but SPP could be equally effective in the protection of adherent HL-60 cells from phorbol ester-induced apoptosis.	transcription
60788	4	336070	5	NULL	NULL	0	NULL	sphingosine	Chemical		does not mediate					apoptosis	Process				NULL	adherent HL-60 cells	0	NULL	NULL	NULL	gw60_jbiolchem_273_25_15345_s_25	9624115	The principal mediator of apoptosis in these cases is ceramide, not sphingosine, but SPP could be equally effective in the protection of adherent HL-60 cells from phorbol ester-induced apoptosis.	transcription
67482	1	336070	7	NULL	NULL	0	NULL	 ceramide	Chemical		mediate					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_25_15345_s_25	9624115	The principal mediator of apoptosis in these cases is ceramide, not sphingosine, but SPP could be equally effective in the protection of adherent HL-60 cells from phorbol ester-induced apoptosis.	transcription
67483	2	336070	7	NULL	NULL	0	NULL	sphingosine	Chemical		does not mediate					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_25_15345_s_25	9624115	The principal mediator of apoptosis in these cases is ceramide, not sphingosine, but SPP could be equally effective in the protection of adherent HL-60 cells from phorbol ester-induced apoptosis.	transcription
67484	3	336070	7	NULL	NULL	0	NULL	phorbol ester	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_25_15345_s_25	9624115	The principal mediator of apoptosis in these cases is ceramide, not sphingosine, but SPP could be equally effective in the protection of adherent HL-60 cells from phorbol ester-induced apoptosis.	transcription
67485	4	336070	7	NULL	NULL	0	NULL	SPP	Chemical		protect					adherent HL-60 cells	Cell				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_25_15345_s_25	9624115	The principal mediator of apoptosis in these cases is ceramide, not sphingosine, but SPP could be equally effective in the protection of adherent HL-60 cells from phorbol ester-induced apoptosis.	transcription
67486	5	336070	7	NULL	NULL	0	NULL	statement 4	Process		protected from					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_25_15345_s_25	9624115	The principal mediator of apoptosis in these cases is ceramide, not sphingosine, but SPP could be equally effective in the protection of adherent HL-60 cells from phorbol ester-induced apoptosis.	transcription
60793	1	336071	5	NULL	NULL	0	NULL	ceramide	Chemical		is a metabolite of					sphingolipid	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_20_12558_s_22	9575216	The sphingolipid metabolite ceramide has been implicated as a stimulator of PKC-inactivating phosphatase catalysis ( 12), and the related metabolite sphingosine is a reversible inhibitor of PKC ( 13).	transcription
60794	2	336071	5	NULL	NULL	0	NULL	PKC	GP		inactivates					phosphatase	GP	catalysis of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_20_12558_s_22	9575216	The sphingolipid metabolite ceramide has been implicated as a stimulator of PKC-inactivating phosphatase catalysis ( 12), and the related metabolite sphingosine is a reversible inhibitor of PKC ( 13).	transcription
60795	3	336071	5	NULL	NULL	0	NULL	ceramide	Chemical		stimulates					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_20_12558_s_22	9575216	The sphingolipid metabolite ceramide has been implicated as a stimulator of PKC-inactivating phosphatase catalysis ( 12), and the related metabolite sphingosine is a reversible inhibitor of PKC ( 13).	transcription
60796	4	336071	5	NULL	NULL	0	NULL	sphingosine	GP		is a reversible inhibitor of					PKC	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_20_12558_s_22	9575216	The sphingolipid metabolite ceramide has been implicated as a stimulator of PKC-inactivating phosphatase catalysis ( 12), and the related metabolite sphingosine is a reversible inhibitor of PKC ( 13).	transcription
67487	1	336071	7	NULL	NULL	0	NULL	ceramide	Chemical		stimulate					PKC-inactivating phosphatase catalysis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_20_12558_s_22	9575216	The sphingolipid metabolite ceramide has been implicated as a stimulator of PKC-inactivating phosphatase catalysis ( 12), and the related metabolite sphingosine is a reversible inhibitor of PKC ( 13).	transcription
67488	2	336071	7	NULL	NULL	0	NULL	sphingosine	Chemical		inhibit		reversibly			PKC	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_20_12558_s_22	9575216	The sphingolipid metabolite ceramide has been implicated as a stimulator of PKC-inactivating phosphatase catalysis ( 12), and the related metabolite sphingosine is a reversible inhibitor of PKC ( 13).	transcription
67489	3	336071	7	NULL	NULL	0	NULL	ceramide	Chemical		is a type of					sphingolipid metabolite	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_20_12558_s_22	9575216	The sphingolipid metabolite ceramide has been implicated as a stimulator of PKC-inactivating phosphatase catalysis ( 12), and the related metabolite sphingosine is a reversible inhibitor of PKC ( 13).	transcription
60797	1	336072	5	NULL	NULL	0	NULL	TNFalpha	GP		induce					apoptosis	Process				NULL	cardiomyocytes	0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_174	8981934	This study provides the first evidence that TNFalpha and its sphingolipid second messenger molecules, including ceramide, sphingosine, and sphingosine-1-phosphate, can induce apoptosis  in cardiomyocytes.	transcription
60798	2	336072	5	NULL	NULL	0	NULL	ceramide	Chemical		induce					apoptosis	Process				NULL	cardiomyocytes	0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_174	8981934	This study provides the first evidence that TNFalpha and its sphingolipid second messenger molecules, including ceramide, sphingosine, and sphingosine-1-phosphate, can induce apoptosis  in cardiomyocytes.	transcription
60800	3	336072	5	NULL	NULL	0	NULL	sphingosine	Chemical		induce					apoptosis	Process				NULL	cardiomyocytes	0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_174	8981934	This study provides the first evidence that TNFalpha and its sphingolipid second messenger molecules, including ceramide, sphingosine, and sphingosine-1-phosphate, can induce apoptosis  in cardiomyocytes.	transcription
60801	4	336072	5	NULL	NULL	0	NULL	sphingosine 1-phosphate	Chemical		induce					apoptosis	Process				NULL	cardiomyocytes	0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_174	8981934	This study provides the first evidence that TNFalpha and its sphingolipid second messenger molecules, including ceramide, sphingosine, and sphingosine-1-phosphate, can induce apoptosis  in cardiomyocytes.	transcription
60802	5	336072	5	NULL	NULL	0	NULL	ceramide	Chemical		is a type of					sphingolipid second messenger molecule	Chemical				NULL		0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_174	8981934	This study provides the first evidence that TNFalpha and its sphingolipid second messenger molecules, including ceramide, sphingosine, and sphingosine-1-phosphate, can induce apoptosis  in cardiomyocytes.	transcription
60803	6	336072	5	NULL	NULL	0	NULL	sphingosine	Chemical		is a type of					sphingolipid second messenger molecule	Chemical				NULL		0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_174	8981934	This study provides the first evidence that TNFalpha and its sphingolipid second messenger molecules, including ceramide, sphingosine, and sphingosine-1-phosphate, can induce apoptosis  in cardiomyocytes.	transcription
60804	7	336072	5	NULL	NULL	0	NULL	sphingosine 1-phosphate	Chemical		is a type of					sphingolipid second messenger molecule	Chemical				NULL		0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_174	8981934	This study provides the first evidence that TNFalpha and its sphingolipid second messenger molecules, including ceramide, sphingosine, and sphingosine-1-phosphate, can induce apoptosis  in cardiomyocytes.	transcription
67490	1	336072	7	NULL	NULL	0	NULL	TNFalpha	GP		induce					apoptosis	Process				NULL	cardiomyocytes	0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_174	8981934	This study provides the first evidence that TNFalpha and its sphingolipid second messenger molecules, including ceramide, sphingosine, and sphingosine-1-phosphate, can induce apoptosis  in cardiomyocytes.	transcription
67491	2	336072	7	NULL	NULL	0	NULL	ceramide	Chemical		induce					apoptosis	Process				NULL	cardiomyocytes	0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_174	8981934	This study provides the first evidence that TNFalpha and its sphingolipid second messenger molecules, including ceramide, sphingosine, and sphingosine-1-phosphate, can induce apoptosis  in cardiomyocytes.	transcription
67492	3	336072	7	NULL	NULL	0	NULL	sphingosine	Chemical		induce					apoptosis	Process				NULL	cardiomyocytes	0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_174	8981934	This study provides the first evidence that TNFalpha and its sphingolipid second messenger molecules, including ceramide, sphingosine, and sphingosine-1-phosphate, can induce apoptosis  in cardiomyocytes.	transcription
67493	4	336072	7	NULL	NULL	NULL	NULL	sphingosine-1-phosphate	Chemical		induce					apoptosis	Process				NULL	cardiomyocytes	NULL	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_174	8981934	This study provides the first evidence that TNFalpha and its sphingolipid second messenger molecules, including ceramide, sphingosine, and sphingosine-1-phosphate, can induce apoptosis  in cardiomyocytes.	transcription
67494	5	336072	7	NULL	NULL	0	NULL	ceramide	Chemical		is a type of					sphingolipid second messenger molecule	Chemical				NULL		0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_174	8981934	This study provides the first evidence that TNFalpha and its sphingolipid second messenger molecules, including ceramide, sphingosine, and sphingosine-1-phosphate, can induce apoptosis  in cardiomyocytes.	transcription
67495	6	336072	7	NULL	NULL	0	NULL	sphingosine	Chemical		is a type of					sphingolipid second messenger molecule	Chemical				NULL		0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_174	8981934	This study provides the first evidence that TNFalpha and its sphingolipid second messenger molecules, including ceramide, sphingosine, and sphingosine-1-phosphate, can induce apoptosis  in cardiomyocytes.	transcription
67496	7	336072	7	NULL	NULL	0	NULL	sphingosine-1-phosphate	Chemical		is a type of					sphingolipid second messenger molecule	Chemical				NULL		0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_174	8981934	This study provides the first evidence that TNFalpha and its sphingolipid second messenger molecules, including ceramide, sphingosine, and sphingosine-1-phosphate, can induce apoptosis  in cardiomyocytes.	transcription
60805	1	336073	5	NULL	NULL	0	NULL	apoptosis	Process		is dependent on					SAPK/AP1	GP				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_8	10454518	In parallel trials, the lethal actions of ceramide (but not of sphingosine) were markedly diminished by pretreatment with diferuloylmethane or expression of TAM-67, confirming the effectiveness of these interventions in suppression of SAPK/AP1-dependent apoptosis.	transcription
60806	2	336073	5	NULL	NULL	0	NULL	diferuloylmethane	Chemical	pretreatment with	diminishes					ceramide	Chemical	lethal actions of			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_8	10454518	In parallel trials, the lethal actions of ceramide (but not of sphingosine) were markedly diminished by pretreatment with diferuloylmethane or expression of TAM-67, confirming the effectiveness of these interventions in suppression of SAPK/AP1-dependent apoptosis.	transcription
60807	3	336073	5	NULL	NULL	0	NULL	TAM-67	GP	expression of	diminishes					ceramide	Chemical	lethal actions of			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_8	10454518	In parallel trials, the lethal actions of ceramide (but not of sphingosine) were markedly diminished by pretreatment with diferuloylmethane or expression of TAM-67, confirming the effectiveness of these interventions in suppression of SAPK/AP1-dependent apoptosis.	transcription
60809	4	336073	5	NULL	NULL	0	NULL	statement 2	Process		suppress					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_8	10454518	In parallel trials, the lethal actions of ceramide (but not of sphingosine) were markedly diminished by pretreatment with diferuloylmethane or expression of TAM-67, confirming the effectiveness of these interventions in suppression of SAPK/AP1-dependent apoptosis.	transcription
60810	5	336073	5	NULL	NULL	0	NULL	statement 3	Process		suppress					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_8	10454518	In parallel trials, the lethal actions of ceramide (but not of sphingosine) were markedly diminished by pretreatment with diferuloylmethane or expression of TAM-67, confirming the effectiveness of these interventions in suppression of SAPK/AP1-dependent apoptosis.	transcription
67497	1	336073	7	NULL	NULL	0	NULL	diferuloylmethane	Chemical		diminish					ceramide	Chemical	lethal actions of			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_8	10454518	In parallel trials, the lethal actions of ceramide (but not of sphingosine) were markedly diminished by pretreatment with diferuloylmethane or expression of TAM-67, confirming the effectiveness of these interventions in suppression of SAPK/AP1-dependent apoptosis.	transcription
67498	2	336073	7	NULL	NULL	NULL	NULL	TAM-67	GP	expression of	diminish					ceramide	Chemical	lethal actions of			NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_8	10454518	In parallel trials, the lethal actions of ceramide (but not of sphingosine) were markedly diminished by pretreatment with diferuloylmethane or expression of TAM-67, confirming the effectiveness of these interventions in suppression of SAPK/AP1-dependent apoptosis.	transcription
67499	3	336073	7	NULL	NULL	0	NULL	diferuloylmethane	Chemical		does not diminish					sphingosine	Chemical	lethal actions of			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_8	10454518	In parallel trials, the lethal actions of ceramide (but not of sphingosine) were markedly diminished by pretreatment with diferuloylmethane or expression of TAM-67, confirming the effectiveness of these interventions in suppression of SAPK/AP1-dependent apoptosis.	transcription
67500	4	336073	7	NULL	NULL	0	NULL	TAM-67	GP	expression of	does not diminish					sphingosine	Chemical	lethal actions of			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_8	10454518	In parallel trials, the lethal actions of ceramide (but not of sphingosine) were markedly diminished by pretreatment with diferuloylmethane or expression of TAM-67, confirming the effectiveness of these interventions in suppression of SAPK/AP1-dependent apoptosis.	transcription
67501	5	336073	7	NULL	NULL	0	NULL	apoptosis	Process		depends on					SAPK/AP1	GP				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_8	10454518	In parallel trials, the lethal actions of ceramide (but not of sphingosine) were markedly diminished by pretreatment with diferuloylmethane or expression of TAM-67, confirming the effectiveness of these interventions in suppression of SAPK/AP1-dependent apoptosis.	transcription
67502	6	336073	7	NULL	NULL	0	NULL	diferuloylmethane	Chemical		suppress					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_8	10454518	In parallel trials, the lethal actions of ceramide (but not of sphingosine) were markedly diminished by pretreatment with diferuloylmethane or expression of TAM-67, confirming the effectiveness of these interventions in suppression of SAPK/AP1-dependent apoptosis.	transcription
67503	7	336073	7	NULL	NULL	0	NULL	 TAM-67	GP	expression of	suppress					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_8	10454518	In parallel trials, the lethal actions of ceramide (but not of sphingosine) were markedly diminished by pretreatment with diferuloylmethane or expression of TAM-67, confirming the effectiveness of these interventions in suppression of SAPK/AP1-dependent apoptosis.	transcription
60892	1	336074	5	NULL	NULL	0	NULL	sphingosine	Chemical		activates					PLD	GP				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_207	9536027	Sphingosine and S-1-P activate PLD and phosphatidic acid and increase mitogenesis, whereas ceramide inhibits PLD and mitogenesis (Yamada and Sakane, 1993  ; Gomez  et al., 1994  ).	transcription
60893	2	336074	5	NULL	NULL	0	NULL	statement 1	Process		increases					mitogenesis	Process				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_207	9536027	Sphingosine and S-1-P activate PLD and phosphatidic acid and increase mitogenesis, whereas ceramide inhibits PLD and mitogenesis (Yamada and Sakane, 1993  ; Gomez  et al., 1994  ).	transcription
60894	3	336074	5	NULL	NULL	0	NULL	sphingosine	Chemical		activates					phosphatidic acid	Chemical				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_207	9536027	Sphingosine and S-1-P activate PLD and phosphatidic acid and increase mitogenesis, whereas ceramide inhibits PLD and mitogenesis (Yamada and Sakane, 1993  ; Gomez  et al., 1994  ).	transcription
60896	4	336074	5	NULL	NULL	0	NULL	statement 3	Process		increases					mitogenesis	Process				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_207	9536027	Sphingosine and S-1-P activate PLD and phosphatidic acid and increase mitogenesis, whereas ceramide inhibits PLD and mitogenesis (Yamada and Sakane, 1993  ; Gomez  et al., 1994  ).	transcription
60897	5	336074	5	NULL	NULL	0	NULL	S-1-P	Chemical		activates					PLD	GP				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_207	9536027	Sphingosine and S-1-P activate PLD and phosphatidic acid and increase mitogenesis, whereas ceramide inhibits PLD and mitogenesis (Yamada and Sakane, 1993  ; Gomez  et al., 1994  ).	transcription
60898	6	336074	5	NULL	NULL	0	NULL	statement 5	Process		increases					mitogenesis	Process				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_207	9536027	Sphingosine and S-1-P activate PLD and phosphatidic acid and increase mitogenesis, whereas ceramide inhibits PLD and mitogenesis (Yamada and Sakane, 1993  ; Gomez  et al., 1994  ).	transcription
60900	7	336074	5	NULL	NULL	0	NULL	S-1-P	Chemical		activates					phosphatidic acid	Chemical				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_207	9536027	Sphingosine and S-1-P activate PLD and phosphatidic acid and increase mitogenesis, whereas ceramide inhibits PLD and mitogenesis (Yamada and Sakane, 1993  ; Gomez  et al., 1994  ).	transcription
60901	8	336074	5	NULL	NULL	0	NULL	statement 7	Process		increases					mitogenesis	Process				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_207	9536027	Sphingosine and S-1-P activate PLD and phosphatidic acid and increase mitogenesis, whereas ceramide inhibits PLD and mitogenesis (Yamada and Sakane, 1993  ; Gomez  et al., 1994  ).	transcription
60903	9	336074	5	NULL	NULL	0	NULL	ceramide	Chemical		inhibits					PLD	GP				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_207	9536027	Sphingosine and S-1-P activate PLD and phosphatidic acid and increase mitogenesis, whereas ceramide inhibits PLD and mitogenesis (Yamada and Sakane, 1993  ; Gomez  et al., 1994  ).	transcription
60904	10	336074	5	NULL	NULL	0	NULL	statement 9	Process		inhibits					mitogenesis	Process				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_207	9536027	Sphingosine and S-1-P activate PLD and phosphatidic acid and increase mitogenesis, whereas ceramide inhibits PLD and mitogenesis (Yamada and Sakane, 1993  ; Gomez  et al., 1994  ).	transcription
67504	1	336074	7	NULL	NULL	0	NULL	Sphingosine	Chemical		activate					PLD	GP				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_207	9536027	Sphingosine and S-1-P activate PLD and phosphatidic acid and increase mitogenesis, whereas ceramide inhibits PLD and mitogenesis (Yamada and Sakane, 1993  ; Gomez  et al., 1994  ).	transcription
67505	2	336074	7	NULL	NULL	0	NULL	S-1-P	Chemical		activate					PLD	GP				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_207	9536027	Sphingosine and S-1-P activate PLD and phosphatidic acid and increase mitogenesis, whereas ceramide inhibits PLD and mitogenesis (Yamada and Sakane, 1993  ; Gomez  et al., 1994  ).	transcription
67506	3	336074	7	NULL	NULL	0	NULL	Sphingosine 	Chemical		activate					phosphatidic acid	Chemical				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_207	9536027	Sphingosine and S-1-P activate PLD and phosphatidic acid and increase mitogenesis, whereas ceramide inhibits PLD and mitogenesis (Yamada and Sakane, 1993  ; Gomez  et al., 1994  ).	transcription
67507	4	336074	7	NULL	NULL	0	NULL	S-1-P	Chemical		activate					phosphatidic acid	Chemical				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_207	9536027	Sphingosine and S-1-P activate PLD and phosphatidic acid and increase mitogenesis, whereas ceramide inhibits PLD and mitogenesis (Yamada and Sakane, 1993  ; Gomez  et al., 1994  ).	transcription
67508	5	336074	7	NULL	NULL	0	NULL	statement 1	Process		increase					mitogenesis	Process				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_207	9536027	Sphingosine and S-1-P activate PLD and phosphatidic acid and increase mitogenesis, whereas ceramide inhibits PLD and mitogenesis (Yamada and Sakane, 1993  ; Gomez  et al., 1994  ).	transcription
67509	6	336074	7	NULL	NULL	0	NULL	statement 2	Process		increase					mitogenesis	Process				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_207	9536027	Sphingosine and S-1-P activate PLD and phosphatidic acid and increase mitogenesis, whereas ceramide inhibits PLD and mitogenesis (Yamada and Sakane, 1993  ; Gomez  et al., 1994  ).	transcription
67510	7	336074	7	NULL	NULL	0	NULL	statement 3	Process		increase					mitogenesis	Process				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_207	9536027	Sphingosine and S-1-P activate PLD and phosphatidic acid and increase mitogenesis, whereas ceramide inhibits PLD and mitogenesis (Yamada and Sakane, 1993  ; Gomez  et al., 1994  ).	transcription
67511	8	336074	7	NULL	NULL	0	NULL	statement 4	Process		increase					mitogenesis	Process				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_207	9536027	Sphingosine and S-1-P activate PLD and phosphatidic acid and increase mitogenesis, whereas ceramide inhibits PLD and mitogenesis (Yamada and Sakane, 1993  ; Gomez  et al., 1994  ).	transcription
67512	9	336074	7	NULL	NULL	0	NULL	ceramide	Chemical		inhibit					PLD	GP				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_207	9536027	Sphingosine and S-1-P activate PLD and phosphatidic acid and increase mitogenesis, whereas ceramide inhibits PLD and mitogenesis (Yamada and Sakane, 1993  ; Gomez  et al., 1994  ).	transcription
67513	10	336074	7	NULL	NULL	0	NULL	ceramide	Chemical		inhibit					mitogenesis	Process				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_285_1_317_s_207	9536027	Sphingosine and S-1-P activate PLD and phosphatidic acid and increase mitogenesis, whereas ceramide inhibits PLD and mitogenesis (Yamada and Sakane, 1993  ; Gomez  et al., 1994  ).	transcription
60911	1	336075	5	NULL	NULL	0	NULL	inflammatory cytokines	GP		stimulates					sphingomyelinase	GP				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochemistry-(mosc)_63_1_9526097_s_5	9526097	Inflammatory cytokines stimulate sphingomyelinase,  but not ceramidase, leading to accumulation of ceramide, whereas growth  signals also stimulate ceramidase and sphingosine kinase leading to increased  SPP levels.	transcription
60912	2	336075	5	NULL	NULL	0	NULL	Inflammatory cytokines	GP		does not stimulate					ceramidase	GP				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochemistry-(mosc)_63_1_9526097_s_5	9526097	Inflammatory cytokines stimulate sphingomyelinase,  but not ceramidase, leading to accumulation of ceramide, whereas growth  signals also stimulate ceramidase and sphingosine kinase leading to increased  SPP levels.	transcription
60913	3	336075	5	NULL	NULL	0	NULL	statement 2	Process		accumulates					ceramide	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochemistry-(mosc)_63_1_9526097_s_5	9526097	Inflammatory cytokines stimulate sphingomyelinase,  but not ceramidase, leading to accumulation of ceramide, whereas growth  signals also stimulate ceramidase and sphingosine kinase leading to increased  SPP levels.	transcription
60915	4	336075	5	NULL	NULL	0	NULL	growth signals	GP		stimulates					ceramidase	GP				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochemistry-(mosc)_63_1_9526097_s_5	9526097	Inflammatory cytokines stimulate sphingomyelinase,  but not ceramidase, leading to accumulation of ceramide, whereas growth  signals also stimulate ceramidase and sphingosine kinase leading to increased  SPP levels.	transcription
60916	5	336075	5	NULL	NULL	0	NULL	statement 4	Process		increases					SPP	Chemical	level of			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochemistry-(mosc)_63_1_9526097_s_5	9526097	Inflammatory cytokines stimulate sphingomyelinase,  but not ceramidase, leading to accumulation of ceramide, whereas growth  signals also stimulate ceramidase and sphingosine kinase leading to increased  SPP levels.	transcription
60917	6	336075	5	NULL	NULL	0	NULL	growth signals	GP		stimulates					sphingosine kinase	GP				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochemistry-(mosc)_63_1_9526097_s_5	9526097	Inflammatory cytokines stimulate sphingomyelinase,  but not ceramidase, leading to accumulation of ceramide, whereas growth  signals also stimulate ceramidase and sphingosine kinase leading to increased  SPP levels.	transcription
60919	7	336075	5	NULL	NULL	0	NULL	statement 6	Process		increases					SPP	Chemical	level of			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochemistry-(mosc)_63_1_9526097_s_5	9526097	Inflammatory cytokines stimulate sphingomyelinase,  but not ceramidase, leading to accumulation of ceramide, whereas growth  signals also stimulate ceramidase and sphingosine kinase leading to increased  SPP levels.	transcription
67514	1	336075	7	NULL	NULL	0	NULL	Inflammatory cytokines 	GP		stimulate					sphingomyelinase	GP				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochemistry-(mosc)_63_1_9526097_s_5	9526097	Inflammatory cytokines stimulate sphingomyelinase,  but not ceramidase, leading to accumulation of ceramide, whereas growth  signals also stimulate ceramidase and sphingosine kinase leading to increased  SPP levels.	transcription
67515	2	336075	7	NULL	NULL	0	NULL	Inflammatory cytokines	GP		does not stimulate					ceramidase	GP				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochemistry-(mosc)_63_1_9526097_s_5	9526097	Inflammatory cytokines stimulate sphingomyelinase,  but not ceramidase, leading to accumulation of ceramide, whereas growth  signals also stimulate ceramidase and sphingosine kinase leading to increased  SPP levels.	transcription
67516	3	336075	7	NULL	NULL	0	NULL	statement 2	Process		leads to					ceramide	Chemical	accumulation of			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochemistry-(mosc)_63_1_9526097_s_5	9526097	Inflammatory cytokines stimulate sphingomyelinase,  but not ceramidase, leading to accumulation of ceramide, whereas growth  signals also stimulate ceramidase and sphingosine kinase leading to increased  SPP levels.	transcription
67517	4	336075	7	NULL	NULL	0	NULL	growth signals	GP		stimulate					ceramidase	GP				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochemistry-(mosc)_63_1_9526097_s_5	9526097	Inflammatory cytokines stimulate sphingomyelinase,  but not ceramidase, leading to accumulation of ceramide, whereas growth  signals also stimulate ceramidase and sphingosine kinase leading to increased  SPP levels.	transcription
67518	5	336075	7	NULL	NULL	0	NULL	growth signals	GP		stimulate					sphingosine kinase 	GP				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochemistry-(mosc)_63_1_9526097_s_5	9526097	Inflammatory cytokines stimulate sphingomyelinase,  but not ceramidase, leading to accumulation of ceramide, whereas growth  signals also stimulate ceramidase and sphingosine kinase leading to increased  SPP levels.	transcription
67519	6	336075	7	NULL	NULL	0	NULL	statement 4	Process		leads to					SPP	Chemical	increased levels of			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochemistry-(mosc)_63_1_9526097_s_5	9526097	Inflammatory cytokines stimulate sphingomyelinase,  but not ceramidase, leading to accumulation of ceramide, whereas growth  signals also stimulate ceramidase and sphingosine kinase leading to increased  SPP levels.	transcription
67520	7	336075	7	NULL	NULL	0	NULL	statement 5	Process		leads to					SPP	Chemical	increased levels of			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochemistry-(mosc)_63_1_9526097_s_5	9526097	Inflammatory cytokines stimulate sphingomyelinase,  but not ceramidase, leading to accumulation of ceramide, whereas growth  signals also stimulate ceramidase and sphingosine kinase leading to increased  SPP levels.	transcription
61011	1	336076	5	NULL	NULL	0	NULL	lipid	Chemical		mediates					cytotoxicity	Process				NULL	U937 cells	0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_156	9415703	View this table:   [in this window]   [in a new window]     [[ TABLE 3        Selectivity ]] of lipid-mediated cytotoxicity in U937 cells    U937 cells were exposed to ceramide or sphingosine at equimolar levels (10 muM) in the presence of the ceramide acylhydrolase inhibitor oleoylethanolamine (100 muM) or the ceramide synthase inhibitor fumonisin B1 (100 muM).	transcription
61012	2	336076	5	NULL	NULL	0	NULL	oleoylethanolamine	Chemical		is an inhibitor of					ceramide acylhydrolase	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_156	9415703	View this table:   [in this window]   [in a new window]     [[ TABLE 3        Selectivity ]] of lipid-mediated cytotoxicity in U937 cells    U937 cells were exposed to ceramide or sphingosine at equimolar levels (10 muM) in the presence of the ceramide acylhydrolase inhibitor oleoylethanolamine (100 muM) or the ceramide synthase inhibitor fumonisin B1 (100 muM).	transcription
61013	3	336076	5	NULL	NULL	0	NULL	fumonisin B1	Chemical		is an inhibitor of					ceramide synthase	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_156	9415703	View this table:   [in this window]   [in a new window]     [[ TABLE 3        Selectivity ]] of lipid-mediated cytotoxicity in U937 cells    U937 cells were exposed to ceramide or sphingosine at equimolar levels (10 muM) in the presence of the ceramide acylhydrolase inhibitor oleoylethanolamine (100 muM) or the ceramide synthase inhibitor fumonisin B1 (100 muM).	transcription
67521	1	336076	7	NULL	NULL	0	NULL	lipid	Chemical		mediate					cytotoxicity	Process				NULL	U937 cells	0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_156	9415703	View this table:   [in this window]   [in a new window]     [[ TABLE 3        Selectivity ]] of lipid-mediated cytotoxicity in U937 cells    U937 cells were exposed to ceramide or sphingosine at equimolar levels (10 muM) in the presence of the ceramide acylhydrolase inhibitor oleoylethanolamine (100 muM) or the ceramide synthase inhibitor fumonisin B1 (100 muM).	transcription
67522	2	336076	7	NULL	NULL	0	NULL	oleoylethanolamine	Chemical		is a type of					ceramide acylhydrolase inhibitor	Chemical				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_156	9415703	View this table:   [in this window]   [in a new window]     [[ TABLE 3        Selectivity ]] of lipid-mediated cytotoxicity in U937 cells    U937 cells were exposed to ceramide or sphingosine at equimolar levels (10 muM) in the presence of the ceramide acylhydrolase inhibitor oleoylethanolamine (100 muM) or the ceramide synthase inhibitor fumonisin B1 (100 muM).	transcription
67523	3	336076	7	NULL	NULL	0	NULL	fumonisin B1	Chemical		is a type of					 ceramide synthase inhibitor	Chemical				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_156	9415703	View this table:   [in this window]   [in a new window]     [[ TABLE 3        Selectivity ]] of lipid-mediated cytotoxicity in U937 cells    U937 cells were exposed to ceramide or sphingosine at equimolar levels (10 muM) in the presence of the ceramide acylhydrolase inhibitor oleoylethanolamine (100 muM) or the ceramide synthase inhibitor fumonisin B1 (100 muM).	transcription
61014	1	336077	5	NULL	NULL	0	NULL	K562 cells	Cell	death of	is induced by					ceramide	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_38_22625_s_141	7545682	To test whether Abl could protect against  ceramide-induced death, K562 cells were exposed to various  concentrations of  N-hexanoyl sphingosine  (C -ceramide), a synthetic cell-permeable ceramide analogue,  and were assessed for apoptosis by flow cytometric analysis.	transcription
61015	2	336077	5	NULL	NULL	0	NULL	Abl	GP		protects against		potentially			statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_38_22625_s_141	7545682	To test whether Abl could protect against  ceramide-induced death, K562 cells were exposed to various  concentrations of  N-hexanoyl sphingosine  (C -ceramide), a synthetic cell-permeable ceramide analogue,  and were assessed for apoptosis by flow cytometric analysis.	transcription
67524	1	336077	7	NULL	NULL	0	NULL	ceramide	Chemical		induce					death	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_38_22625_s_141	7545682	To test whether Abl could protect against  ceramide-induced death, K562 cells were exposed to various  concentrations of  N-hexanoyl sphingosine  (C -ceramide), a synthetic cell-permeable ceramide analogue,  and were assessed for apoptosis by flow cytometric analysis.	transcription
67525	2	336077	7	NULL	NULL	0	NULL	N-hexanoyl sphingosine	Chemical		is a type of					synthetic cell-permeable ceramide analogue	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_38_22625_s_141	7545682	To test whether Abl could protect against  ceramide-induced death, K562 cells were exposed to various  concentrations of  N-hexanoyl sphingosine  (C -ceramide), a synthetic cell-permeable ceramide analogue,  and were assessed for apoptosis by flow cytometric analysis.	transcription
67526	3	336077	7	NULL	NULL	0	NULL	N-hexanoyl sphingosine	Chemical		is					C -ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_38_22625_s_141	7545682	To test whether Abl could protect against  ceramide-induced death, K562 cells were exposed to various  concentrations of  N-hexanoyl sphingosine  (C -ceramide), a synthetic cell-permeable ceramide analogue,  and were assessed for apoptosis by flow cytometric analysis.	transcription
61016	1	336078	5	NULL	NULL	0	NULL	OE	Chemical		is					oleoylethanolamine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2591_s_155	9446561	After 24 h of incubation, concentration of nitrite was measured in the supernatants as mentioned under     Oleoylethanolamine (OE), an inhibitor of ceramidase, the enzyme responsible for the catabolism of ceramide to sphingosine and fatty acid, has been reported to induce apoptosis in neuroblastoma cells ( 23) because of the increased concentration of ceramide due to the inhibition of catabolism of ceramide ( 23).	transcription
61017	2	336078	5	NULL	NULL	0	NULL	oleoylethanolamine	Chemical		is an inhibitor of					ceramidase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2591_s_155	9446561	After 24 h of incubation, concentration of nitrite was measured in the supernatants as mentioned under     Oleoylethanolamine (OE), an inhibitor of ceramidase, the enzyme responsible for the catabolism of ceramide to sphingosine and fatty acid, has been reported to induce apoptosis in neuroblastoma cells ( 23) because of the increased concentration of ceramide due to the inhibition of catabolism of ceramide ( 23).	transcription
61018	3	336078	5	NULL	NULL	0	NULL	ceramide	Chemical		is catabolised to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2591_s_155	9446561	After 24 h of incubation, concentration of nitrite was measured in the supernatants as mentioned under     Oleoylethanolamine (OE), an inhibitor of ceramidase, the enzyme responsible for the catabolism of ceramide to sphingosine and fatty acid, has been reported to induce apoptosis in neuroblastoma cells ( 23) because of the increased concentration of ceramide due to the inhibition of catabolism of ceramide ( 23).	transcription
61019	4	336078	5	NULL	NULL	0	NULL	ceramide	Chemical		is catabolised to					fatty acid	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2591_s_155	9446561	After 24 h of incubation, concentration of nitrite was measured in the supernatants as mentioned under     Oleoylethanolamine (OE), an inhibitor of ceramidase, the enzyme responsible for the catabolism of ceramide to sphingosine and fatty acid, has been reported to induce apoptosis in neuroblastoma cells ( 23) because of the increased concentration of ceramide due to the inhibition of catabolism of ceramide ( 23).	transcription
61020	5	336078	5	NULL	NULL	0	NULL	statement 3	Process		occurs along with					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2591_s_155	9446561	After 24 h of incubation, concentration of nitrite was measured in the supernatants as mentioned under     Oleoylethanolamine (OE), an inhibitor of ceramidase, the enzyme responsible for the catabolism of ceramide to sphingosine and fatty acid, has been reported to induce apoptosis in neuroblastoma cells ( 23) because of the increased concentration of ceramide due to the inhibition of catabolism of ceramide ( 23).	transcription
61021	6	336078	5	NULL	NULL	0	NULL	ceramidase	GP		catalyzes					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2591_s_155	9446561	After 24 h of incubation, concentration of nitrite was measured in the supernatants as mentioned under     Oleoylethanolamine (OE), an inhibitor of ceramidase, the enzyme responsible for the catabolism of ceramide to sphingosine and fatty acid, has been reported to induce apoptosis in neuroblastoma cells ( 23) because of the increased concentration of ceramide due to the inhibition of catabolism of ceramide ( 23).	transcription
61022	7	336078	5	NULL	NULL	0	NULL	oleoylethanolamine	Chemical		induce					apoptosis	Process				NULL	neuroblastoma cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_5_2591_s_155	9446561	After 24 h of incubation, concentration of nitrite was measured in the supernatants as mentioned under     Oleoylethanolamine (OE), an inhibitor of ceramidase, the enzyme responsible for the catabolism of ceramide to sphingosine and fatty acid, has been reported to induce apoptosis in neuroblastoma cells ( 23) because of the increased concentration of ceramide due to the inhibition of catabolism of ceramide ( 23).	transcription
61023	8	336078	5	NULL	NULL	0	NULL	ceramide	Chemical	inhibition of;;catabolism of	increases					ceramide	Chemical	concentration of			NULL	neuroblastoma cells	0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2591_s_155	9446561	After 24 h of incubation, concentration of nitrite was measured in the supernatants as mentioned under     Oleoylethanolamine (OE), an inhibitor of ceramidase, the enzyme responsible for the catabolism of ceramide to sphingosine and fatty acid, has been reported to induce apoptosis in neuroblastoma cells ( 23) because of the increased concentration of ceramide due to the inhibition of catabolism of ceramide ( 23).	transcription
61024	9	336078	5	NULL	NULL	0	NULL	statement 8	Process		leads to					statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2591_s_155	9446561	After 24 h of incubation, concentration of nitrite was measured in the supernatants as mentioned under     Oleoylethanolamine (OE), an inhibitor of ceramidase, the enzyme responsible for the catabolism of ceramide to sphingosine and fatty acid, has been reported to induce apoptosis in neuroblastoma cells ( 23) because of the increased concentration of ceramide due to the inhibition of catabolism of ceramide ( 23).	transcription
67527	1	336078	7	NULL	NULL	0	NULL	ceramide	Chemical		catabolized to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2591_s_155	9446561	After 24 h of incubation, concentration of nitrite was measured in the supernatants as mentioned under     Oleoylethanolamine (OE), an inhibitor of ceramidase, the enzyme responsible for the catabolism of ceramide to sphingosine and fatty acid, has been reported to induce apoptosis in neuroblastoma cells ( 23) because of the increased concentration of ceramide due to the inhibition of catabolism of ceramide ( 23).	transcription
67528	2	336078	7	NULL	NULL	0	NULL	ceramide	Chemical		catabolized to					fatty acid	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2591_s_155	9446561	After 24 h of incubation, concentration of nitrite was measured in the supernatants as mentioned under     Oleoylethanolamine (OE), an inhibitor of ceramidase, the enzyme responsible for the catabolism of ceramide to sphingosine and fatty acid, has been reported to induce apoptosis in neuroblastoma cells ( 23) because of the increased concentration of ceramide due to the inhibition of catabolism of ceramide ( 23).	transcription
67529	3	336078	7	NULL	NULL	0	NULL	statement 1	Process		occur along with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2591_s_155	9446561	After 24 h of incubation, concentration of nitrite was measured in the supernatants as mentioned under     Oleoylethanolamine (OE), an inhibitor of ceramidase, the enzyme responsible for the catabolism of ceramide to sphingosine and fatty acid, has been reported to induce apoptosis in neuroblastoma cells ( 23) because of the increased concentration of ceramide due to the inhibition of catabolism of ceramide ( 23).	transcription
67530	4	336078	7	NULL	NULL	0	NULL	ceramidase	GP		catalyze					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2591_s_155	9446561	After 24 h of incubation, concentration of nitrite was measured in the supernatants as mentioned under     Oleoylethanolamine (OE), an inhibitor of ceramidase, the enzyme responsible for the catabolism of ceramide to sphingosine and fatty acid, has been reported to induce apoptosis in neuroblastoma cells ( 23) because of the increased concentration of ceramide due to the inhibition of catabolism of ceramide ( 23).	transcription
67531	5	336078	7	NULL	NULL	0	NULL	OE	Chemical		is an inhibitor of					ceramidase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2591_s_155	9446561	After 24 h of incubation, concentration of nitrite was measured in the supernatants as mentioned under     Oleoylethanolamine (OE), an inhibitor of ceramidase, the enzyme responsible for the catabolism of ceramide to sphingosine and fatty acid, has been reported to induce apoptosis in neuroblastoma cells ( 23) because of the increased concentration of ceramide due to the inhibition of catabolism of ceramide ( 23).	transcription
67532	6	336078	7	NULL	NULL	0	NULL	OE	Chemical		is					Oleoylethanolamine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2591_s_155	9446561	After 24 h of incubation, concentration of nitrite was measured in the supernatants as mentioned under     Oleoylethanolamine (OE), an inhibitor of ceramidase, the enzyme responsible for the catabolism of ceramide to sphingosine and fatty acid, has been reported to induce apoptosis in neuroblastoma cells ( 23) because of the increased concentration of ceramide due to the inhibition of catabolism of ceramide ( 23).	transcription
67533	7	336078	7	NULL	NULL	0	NULL	statement 3	Process		induce					apoptosis	Process				NULL	neuroblastoma cells	0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2591_s_155	9446561	After 24 h of incubation, concentration of nitrite was measured in the supernatants as mentioned under     Oleoylethanolamine (OE), an inhibitor of ceramidase, the enzyme responsible for the catabolism of ceramide to sphingosine and fatty acid, has been reported to induce apoptosis in neuroblastoma cells ( 23) because of the increased concentration of ceramide due to the inhibition of catabolism of ceramide ( 23).	transcription
67534	8	336078	7	NULL	NULL	0	NULL	statement 7	Process		because of					ceramide 	Chemical	increased concentration of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2591_s_155	9446561	After 24 h of incubation, concentration of nitrite was measured in the supernatants as mentioned under     Oleoylethanolamine (OE), an inhibitor of ceramidase, the enzyme responsible for the catabolism of ceramide to sphingosine and fatty acid, has been reported to induce apoptosis in neuroblastoma cells ( 23) because of the increased concentration of ceramide due to the inhibition of catabolism of ceramide ( 23).	transcription
61025	1	336079	5	NULL	NULL	0	NULL	SPP	Chemical		is					sphingosine 1-phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_3	9446602	A further metabolite of ceramide, sphingosine 1-phosphate (SPP), prevents ceramide-mediated apoptosis, and it has been suggested that the balance between intracellular ceramide and SPP levels may determine the cell fate (Cuvillier, O., Pirianov, G, Kleuser, B., Vanek, P. G., Coso, O.	transcription
61026	2	336079	5	NULL	NULL	0	NULL	SPP	Chemical		is a metabolite of					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_3	9446602	A further metabolite of ceramide, sphingosine 1-phosphate (SPP), prevents ceramide-mediated apoptosis, and it has been suggested that the balance between intracellular ceramide and SPP levels may determine the cell fate (Cuvillier, O., Pirianov, G, Kleuser, B., Vanek, P. G., Coso, O.	transcription
61027	3	336079	5	NULL	NULL	0	NULL	apoptosis	Process		is mediated by					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_3	9446602	A further metabolite of ceramide, sphingosine 1-phosphate (SPP), prevents ceramide-mediated apoptosis, and it has been suggested that the balance between intracellular ceramide and SPP levels may determine the cell fate (Cuvillier, O., Pirianov, G, Kleuser, B., Vanek, P. G., Coso, O.	transcription
61028	4	336079	5	NULL	NULL	0	NULL	SPP	Chemical		prevents					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_3	9446602	A further metabolite of ceramide, sphingosine 1-phosphate (SPP), prevents ceramide-mediated apoptosis, and it has been suggested that the balance between intracellular ceramide and SPP levels may determine the cell fate (Cuvillier, O., Pirianov, G, Kleuser, B., Vanek, P. G., Coso, O.	transcription
61029	5	336079	5	NULL	NULL	0	NULL	ceramide	Chemical	intracellular levels of	is balanced with					SPP	Chemical	intracellular levels of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_3	9446602	A further metabolite of ceramide, sphingosine 1-phosphate (SPP), prevents ceramide-mediated apoptosis, and it has been suggested that the balance between intracellular ceramide and SPP levels may determine the cell fate (Cuvillier, O., Pirianov, G, Kleuser, B., Vanek, P. G., Coso, O.	transcription
61030	6	336079	5	NULL	NULL	0	NULL	statement 5	Process		determines		may			cell fate	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_3	9446602	A further metabolite of ceramide, sphingosine 1-phosphate (SPP), prevents ceramide-mediated apoptosis, and it has been suggested that the balance between intracellular ceramide and SPP levels may determine the cell fate (Cuvillier, O., Pirianov, G, Kleuser, B., Vanek, P. G., Coso, O.	transcription
67535	1	336079	7	NULL	NULL	0	NULL	ceramide	Chemical		mediate					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_3	9446602	A further metabolite of ceramide, sphingosine 1-phosphate (SPP), prevents ceramide-mediated apoptosis, and it has been suggested that the balance between intracellular ceramide and SPP levels may determine the cell fate (Cuvillier, O., Pirianov, G, Kleuser, B., Vanek, P. G., Coso, O.	transcription
67536	2	336079	7	NULL	NULL	0	NULL	SPP	Chemical		prevents					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_3	9446602	A further metabolite of ceramide, sphingosine 1-phosphate (SPP), prevents ceramide-mediated apoptosis, and it has been suggested that the balance between intracellular ceramide and SPP levels may determine the cell fate (Cuvillier, O., Pirianov, G, Kleuser, B., Vanek, P. G., Coso, O.	transcription
67537	3	336079	7	NULL	NULL	0	NULL	SPP	Chemical		is					sphingosine 1-phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_3	9446602	A further metabolite of ceramide, sphingosine 1-phosphate (SPP), prevents ceramide-mediated apoptosis, and it has been suggested that the balance between intracellular ceramide and SPP levels may determine the cell fate (Cuvillier, O., Pirianov, G, Kleuser, B., Vanek, P. G., Coso, O.	transcription
67538	4	336079	7	NULL	NULL	0	NULL	SPP	Chemical		is a metabolite of					ceramide 	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_3	9446602	A further metabolite of ceramide, sphingosine 1-phosphate (SPP), prevents ceramide-mediated apoptosis, and it has been suggested that the balance between intracellular ceramide and SPP levels may determine the cell fate (Cuvillier, O., Pirianov, G, Kleuser, B., Vanek, P. G., Coso, O.	transcription
67539	5	336079	7	NULL	NULL	0	NULL	ceramide	Chemical	intracellular	balanced with					SPP	Chemical	levels of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_3	9446602	A further metabolite of ceramide, sphingosine 1-phosphate (SPP), prevents ceramide-mediated apoptosis, and it has been suggested that the balance between intracellular ceramide and SPP levels may determine the cell fate (Cuvillier, O., Pirianov, G, Kleuser, B., Vanek, P. G., Coso, O.	transcription
67540	6	336079	7	NULL	NULL	0	NULL	statement 5	Process		determine					cell fate	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_3	9446602	A further metabolite of ceramide, sphingosine 1-phosphate (SPP), prevents ceramide-mediated apoptosis, and it has been suggested that the balance between intracellular ceramide and SPP levels may determine the cell fate (Cuvillier, O., Pirianov, G, Kleuser, B., Vanek, P. G., Coso, O.	transcription
61031	1	336080	5	NULL	NULL	0	NULL	progesterone	GP	production of	is induced by					LH	GP				NULL		0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_153	9915989	Since exogenous SMase inhibited LH-induced progesterone production, the abilities of ceramides of different acyl chain length (C2-, C6-, and C8-ceramide) and of sphingosine to inhibit LH (10 ng/ml)-induced progesterone production were also assessed to confirm that the effects of SMase were mediated via ceramide and not through nonspecific actions of the enzyme ( Fig. 4).	transcription
61032	2	336080	5	NULL	NULL	0	NULL	SMase	GP		inhibits					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_153	9915989	Since exogenous SMase inhibited LH-induced progesterone production, the abilities of ceramides of different acyl chain length (C2-, C6-, and C8-ceramide) and of sphingosine to inhibit LH (10 ng/ml)-induced progesterone production were also assessed to confirm that the effects of SMase were mediated via ceramide and not through nonspecific actions of the enzyme ( Fig. 4).	transcription
61033	3	336080	5	NULL	NULL	0	NULL	sphingosine	Chemical		inhibits					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_153	9915989	Since exogenous SMase inhibited LH-induced progesterone production, the abilities of ceramides of different acyl chain length (C2-, C6-, and C8-ceramide) and of sphingosine to inhibit LH (10 ng/ml)-induced progesterone production were also assessed to confirm that the effects of SMase were mediated via ceramide and not through nonspecific actions of the enzyme ( Fig. 4).	transcription
61034	4	336080	5	NULL	NULL	0	NULL	C2-ceramide	Chemical		inhibits					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_153	9915989	Since exogenous SMase inhibited LH-induced progesterone production, the abilities of ceramides of different acyl chain length (C2-, C6-, and C8-ceramide) and of sphingosine to inhibit LH (10 ng/ml)-induced progesterone production were also assessed to confirm that the effects of SMase were mediated via ceramide and not through nonspecific actions of the enzyme ( Fig. 4).	transcription
61035	5	336080	5	NULL	NULL	0	NULL	C6-ceramide	Chemical		inhibits					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_153	9915989	Since exogenous SMase inhibited LH-induced progesterone production, the abilities of ceramides of different acyl chain length (C2-, C6-, and C8-ceramide) and of sphingosine to inhibit LH (10 ng/ml)-induced progesterone production were also assessed to confirm that the effects of SMase were mediated via ceramide and not through nonspecific actions of the enzyme ( Fig. 4).	transcription
61036	6	336080	5	NULL	NULL	0	NULL	C8-ceramide	Chemical		inhibits					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_153	9915989	Since exogenous SMase inhibited LH-induced progesterone production, the abilities of ceramides of different acyl chain length (C2-, C6-, and C8-ceramide) and of sphingosine to inhibit LH (10 ng/ml)-induced progesterone production were also assessed to confirm that the effects of SMase were mediated via ceramide and not through nonspecific actions of the enzyme ( Fig. 4).	transcription
61037	7	336080	5	NULL	NULL	0	NULL	statement 2	Process		via					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_153	9915989	Since exogenous SMase inhibited LH-induced progesterone production, the abilities of ceramides of different acyl chain length (C2-, C6-, and C8-ceramide) and of sphingosine to inhibit LH (10 ng/ml)-induced progesterone production were also assessed to confirm that the effects of SMase were mediated via ceramide and not through nonspecific actions of the enzyme ( Fig. 4).	transcription
67541	1	336080	7	NULL	NULL	0	NULL	 LH	GP		induce					progesterone	Chemical	production of			NULL		0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_153	9915989	Since exogenous SMase inhibited LH-induced progesterone production, the abilities of ceramides of different acyl chain length (C2-, C6-, and C8-ceramide) and of sphingosine to inhibit LH (10 ng/ml)-induced progesterone production were also assessed to confirm that the effects of SMase were mediated via ceramide and not through nonspecific actions of the enzyme ( Fig. 4).	transcription
67542	2	336080	7	NULL	NULL	0	NULL	SMase	GP		inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_153	9915989	Since exogenous SMase inhibited LH-induced progesterone production, the abilities of ceramides of different acyl chain length (C2-, C6-, and C8-ceramide) and of sphingosine to inhibit LH (10 ng/ml)-induced progesterone production were also assessed to confirm that the effects of SMase were mediated via ceramide and not through nonspecific actions of the enzyme ( Fig. 4).	transcription
67543	3	336080	7	NULL	NULL	NULL	NULL	C2-ceramide	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_153	9915989	Since exogenous SMase inhibited LH-induced progesterone production, the abilities of ceramides of different acyl chain length (C2-, C6-, and C8-ceramide) and of sphingosine to inhibit LH (10 ng/ml)-induced progesterone production were also assessed to confirm that the effects of SMase were mediated via ceramide and not through nonspecific actions of the enzyme ( Fig. 4).	transcription
67544	4	336080	7	NULL	NULL	0	NULL	C6-ceramide	Chemical		inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_153	9915989	Since exogenous SMase inhibited LH-induced progesterone production, the abilities of ceramides of different acyl chain length (C2-, C6-, and C8-ceramide) and of sphingosine to inhibit LH (10 ng/ml)-induced progesterone production were also assessed to confirm that the effects of SMase were mediated via ceramide and not through nonspecific actions of the enzyme ( Fig. 4).	transcription
67545	5	336080	7	NULL	NULL	0	NULL	C8-ceramide	Chemical		inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_153	9915989	Since exogenous SMase inhibited LH-induced progesterone production, the abilities of ceramides of different acyl chain length (C2-, C6-, and C8-ceramide) and of sphingosine to inhibit LH (10 ng/ml)-induced progesterone production were also assessed to confirm that the effects of SMase were mediated via ceramide and not through nonspecific actions of the enzyme ( Fig. 4).	transcription
67546	6	336080	7	NULL	NULL	0	NULL	sphingosine	Chemical		inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_153	9915989	Since exogenous SMase inhibited LH-induced progesterone production, the abilities of ceramides of different acyl chain length (C2-, C6-, and C8-ceramide) and of sphingosine to inhibit LH (10 ng/ml)-induced progesterone production were also assessed to confirm that the effects of SMase were mediated via ceramide and not through nonspecific actions of the enzyme ( Fig. 4).	transcription
67547	7	336080	7	NULL	NULL	0	NULL	SMase	GP	effects of	mediated via					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_153	9915989	Since exogenous SMase inhibited LH-induced progesterone production, the abilities of ceramides of different acyl chain length (C2-, C6-, and C8-ceramide) and of sphingosine to inhibit LH (10 ng/ml)-induced progesterone production were also assessed to confirm that the effects of SMase were mediated via ceramide and not through nonspecific actions of the enzyme ( Fig. 4).	transcription
67548	1	336081	7	NULL	NULL	0	NULL	ceramide 	Chemical	short acyl chain analogues of	metabolized to		mainly			GlcCer	Chemical				NULL	fibroblasts	0	NULL	NULL	NULL	gw60_jbiolchem_272_3_1558_s_99	8999828	Since in fibroblasts, short acyl chain analogues of ceramide are metabolized mainly to GlcCer and SM (not shown; see also Meivar-Levy  et al. ( 24)), and since sphinganine, sphingosine, and ceramides do not significantly affect cell morphology, these data together demonstrate that the ability of GM3 to restore cell morphology is due to depletion of an essential higher order glycosphingolipid, probably GM3, and not due to accumulation or depletion of bioactive intermediates.	transcription
67549	2	336081	7	NULL	NULL	0	NULL	ceramide	Chemical	short acyl chain analogues of	metabolized to		mainly			SM	Chemical				NULL	fibroblasts	0	NULL	NULL	NULL	gw60_jbiolchem_272_3_1558_s_99	8999828	Since in fibroblasts, short acyl chain analogues of ceramide are metabolized mainly to GlcCer and SM (not shown; see also Meivar-Levy  et al. ( 24)), and since sphinganine, sphingosine, and ceramides do not significantly affect cell morphology, these data together demonstrate that the ability of GM3 to restore cell morphology is due to depletion of an essential higher order glycosphingolipid, probably GM3, and not due to accumulation or depletion of bioactive intermediates.	transcription
67550	3	336081	7	NULL	NULL	0	NULL	statement 1	Process		occur along with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_3_1558_s_99	8999828	Since in fibroblasts, short acyl chain analogues of ceramide are metabolized mainly to GlcCer and SM (not shown; see also Meivar-Levy  et al. ( 24)), and since sphinganine, sphingosine, and ceramides do not significantly affect cell morphology, these data together demonstrate that the ability of GM3 to restore cell morphology is due to depletion of an essential higher order glycosphingolipid, probably GM3, and not due to accumulation or depletion of bioactive intermediates.	transcription
67551	4	336081	7	NULL	NULL	NULL	NULL	sphinganine	Chemical		does not affect		significantly			cell morphology	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_3_1558_s_99	8999828	Since in fibroblasts, short acyl chain analogues of ceramide are metabolized mainly to GlcCer and SM (not shown; see also Meivar-Levy  et al. ( 24)), and since sphinganine, sphingosine, and ceramides do not significantly affect cell morphology, these data together demonstrate that the ability of GM3 to restore cell morphology is due to depletion of an essential higher order glycosphingolipid, probably GM3, and not due to accumulation or depletion of bioactive intermediates.	transcription
67552	5	336081	7	NULL	NULL	0	NULL	sphingosine	Chemical		does not affect		significantly			cell morphology	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_3_1558_s_99	8999828	Since in fibroblasts, short acyl chain analogues of ceramide are metabolized mainly to GlcCer and SM (not shown; see also Meivar-Levy  et al. ( 24)), and since sphinganine, sphingosine, and ceramides do not significantly affect cell morphology, these data together demonstrate that the ability of GM3 to restore cell morphology is due to depletion of an essential higher order glycosphingolipid, probably GM3, and not due to accumulation or depletion of bioactive intermediates.	transcription
67553	6	336081	7	NULL	NULL	0	NULL	ceramides	Chemical		does not affect		significantly			cell morphology	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_3_1558_s_99	8999828	Since in fibroblasts, short acyl chain analogues of ceramide are metabolized mainly to GlcCer and SM (not shown; see also Meivar-Levy  et al. ( 24)), and since sphinganine, sphingosine, and ceramides do not significantly affect cell morphology, these data together demonstrate that the ability of GM3 to restore cell morphology is due to depletion of an essential higher order glycosphingolipid, probably GM3, and not due to accumulation or depletion of bioactive intermediates.	transcription
67554	7	336081	7	NULL	NULL	0	NULL	GM3	Chemical		restore					cell morphology	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_3_1558_s_99	8999828	Since in fibroblasts, short acyl chain analogues of ceramide are metabolized mainly to GlcCer and SM (not shown; see also Meivar-Levy  et al. ( 24)), and since sphinganine, sphingosine, and ceramides do not significantly affect cell morphology, these data together demonstrate that the ability of GM3 to restore cell morphology is due to depletion of an essential higher order glycosphingolipid, probably GM3, and not due to accumulation or depletion of bioactive intermediates.	transcription
67555	8	336081	7	NULL	NULL	0	NULL	statement 7	Process		due to					GM3	Chemical	depletion of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_3_1558_s_99	8999828	Since in fibroblasts, short acyl chain analogues of ceramide are metabolized mainly to GlcCer and SM (not shown; see also Meivar-Levy  et al. ( 24)), and since sphinganine, sphingosine, and ceramides do not significantly affect cell morphology, these data together demonstrate that the ability of GM3 to restore cell morphology is due to depletion of an essential higher order glycosphingolipid, probably GM3, and not due to accumulation or depletion of bioactive intermediates.	transcription
67556	9	336081	7	NULL	NULL	0	NULL	GM3	Chemical		is a type of					essential higher order glycosphingolipid	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_3_1558_s_99	8999828	Since in fibroblasts, short acyl chain analogues of ceramide are metabolized mainly to GlcCer and SM (not shown; see also Meivar-Levy  et al. ( 24)), and since sphinganine, sphingosine, and ceramides do not significantly affect cell morphology, these data together demonstrate that the ability of GM3 to restore cell morphology is due to depletion of an essential higher order glycosphingolipid, probably GM3, and not due to accumulation or depletion of bioactive intermediates.	transcription
67557	10	336081	7	NULL	NULL	0	NULL	statement 7	Process		not due to					bioactive intermediates	Chemical	accumulation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_3_1558_s_99	8999828	Since in fibroblasts, short acyl chain analogues of ceramide are metabolized mainly to GlcCer and SM (not shown; see also Meivar-Levy  et al. ( 24)), and since sphinganine, sphingosine, and ceramides do not significantly affect cell morphology, these data together demonstrate that the ability of GM3 to restore cell morphology is due to depletion of an essential higher order glycosphingolipid, probably GM3, and not due to accumulation or depletion of bioactive intermediates.	transcription
67558	11	336081	7	NULL	NULL	0	NULL	statement 7	Process		not due to					bioactive intermediates	Chemical	depletion of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_3_1558_s_99	8999828	Since in fibroblasts, short acyl chain analogues of ceramide are metabolized mainly to GlcCer and SM (not shown; see also Meivar-Levy  et al. ( 24)), and since sphinganine, sphingosine, and ceramides do not significantly affect cell morphology, these data together demonstrate that the ability of GM3 to restore cell morphology is due to depletion of an essential higher order glycosphingolipid, probably GM3, and not due to accumulation or depletion of bioactive intermediates.	transcription
61130	1	336082	5	NULL	NULL	0	NULL	sphingosine burst	Process		arise from					complex sphingolipids	Chemical	turnover of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_32_18749_s_6	7642524	In contrast, the sphingosine  burst arose mainly from turnover of complex sphingolipids because no  incorporation of [ H]serine or  [ H]palmitate into sphingosine was detected;  sphingosine mass was not affected by beta-F-alanine or the serine  concentration; and, the burst could be followed by the release of  sphingosine and ceramide from complex sphingolipids (especially  sphingomyelin) in a process that was inhibited by NH Cl and  chloroquine.	transcription
61131	2	336082	5	NULL	NULL	0	NULL	[ H]serine	AminoAcid		not incorporated into					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_32_18749_s_6	7642524	In contrast, the sphingosine  burst arose mainly from turnover of complex sphingolipids because no  incorporation of [ H]serine or  [ H]palmitate into sphingosine was detected;  sphingosine mass was not affected by beta-F-alanine or the serine  concentration; and, the burst could be followed by the release of  sphingosine and ceramide from complex sphingolipids (especially  sphingomyelin) in a process that was inhibited by NH Cl and  chloroquine.	transcription
61132	3	336082	5	NULL	NULL	0	NULL	[ H]palmitate	Chemical		not incorporated into					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_32_18749_s_6	7642524	In contrast, the sphingosine  burst arose mainly from turnover of complex sphingolipids because no  incorporation of [ H]serine or  [ H]palmitate into sphingosine was detected;  sphingosine mass was not affected by beta-F-alanine or the serine  concentration; and, the burst could be followed by the release of  sphingosine and ceramide from complex sphingolipids (especially  sphingomyelin) in a process that was inhibited by NH Cl and  chloroquine.	transcription
61133	4	336082	5	NULL	NULL	0	NULL	sphingosine 	Chemical	mass of	is not affected by					beta-F-alanine	AminoAcid	concentration of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_32_18749_s_6	7642524	In contrast, the sphingosine  burst arose mainly from turnover of complex sphingolipids because no  incorporation of [ H]serine or  [ H]palmitate into sphingosine was detected;  sphingosine mass was not affected by beta-F-alanine or the serine  concentration; and, the burst could be followed by the release of  sphingosine and ceramide from complex sphingolipids (especially  sphingomyelin) in a process that was inhibited by NH Cl and  chloroquine.	transcription
61134	5	336082	5	NULL	NULL	0	NULL	sphingosine	Chemical	mass of	is not affected by					serine	AminoAcid	concentration of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_32_18749_s_6	7642524	In contrast, the sphingosine  burst arose mainly from turnover of complex sphingolipids because no  incorporation of [ H]serine or  [ H]palmitate into sphingosine was detected;  sphingosine mass was not affected by beta-F-alanine or the serine  concentration; and, the burst could be followed by the release of  sphingosine and ceramide from complex sphingolipids (especially  sphingomyelin) in a process that was inhibited by NH Cl and  chloroquine.	transcription
61135	6	336082	5	NULL	NULL	0	NULL	sphingosine	Chemical		is release from					sphingomyelin	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_32_18749_s_6	7642524	In contrast, the sphingosine  burst arose mainly from turnover of complex sphingolipids because no  incorporation of [ H]serine or  [ H]palmitate into sphingosine was detected;  sphingosine mass was not affected by beta-F-alanine or the serine  concentration; and, the burst could be followed by the release of  sphingosine and ceramide from complex sphingolipids (especially  sphingomyelin) in a process that was inhibited by NH Cl and  chloroquine.	transcription
61136	7	336082	5	NULL	NULL	0	NULL	ceramide	Chemical		is release from					sphingomyelin	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_32_18749_s_6	7642524	In contrast, the sphingosine  burst arose mainly from turnover of complex sphingolipids because no  incorporation of [ H]serine or  [ H]palmitate into sphingosine was detected;  sphingosine mass was not affected by beta-F-alanine or the serine  concentration; and, the burst could be followed by the release of  sphingosine and ceramide from complex sphingolipids (especially  sphingomyelin) in a process that was inhibited by NH Cl and  chloroquine.	transcription
61137	8	336082	5	NULL	NULL	0	NULL	sphingomyelin	Chemical		is a type of					complex sphingolipids	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_32_18749_s_6	7642524	In contrast, the sphingosine  burst arose mainly from turnover of complex sphingolipids because no  incorporation of [ H]serine or  [ H]palmitate into sphingosine was detected;  sphingosine mass was not affected by beta-F-alanine or the serine  concentration; and, the burst could be followed by the release of  sphingosine and ceramide from complex sphingolipids (especially  sphingomyelin) in a process that was inhibited by NH Cl and  chloroquine.	transcription
61138	9	336082	5	NULL	NULL	0	NULL	sphingosine burst	Process		followed by					statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_32_18749_s_6	7642524	In contrast, the sphingosine  burst arose mainly from turnover of complex sphingolipids because no  incorporation of [ H]serine or  [ H]palmitate into sphingosine was detected;  sphingosine mass was not affected by beta-F-alanine or the serine  concentration; and, the burst could be followed by the release of  sphingosine and ceramide from complex sphingolipids (especially  sphingomyelin) in a process that was inhibited by NH Cl and  chloroquine.	transcription
61139	10	336082	5	NULL	NULL	0	NULL	sphingosine burst	Process		followed by					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_32_18749_s_6	7642524	In contrast, the sphingosine  burst arose mainly from turnover of complex sphingolipids because no  incorporation of [ H]serine or  [ H]palmitate into sphingosine was detected;  sphingosine mass was not affected by beta-F-alanine or the serine  concentration; and, the burst could be followed by the release of  sphingosine and ceramide from complex sphingolipids (especially  sphingomyelin) in a process that was inhibited by NH Cl and  chloroquine.	transcription
61140	11	336082	5	NULL	NULL	0	NULL	statement 9	Process		is inhibited by					NH Cl	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_32_18749_s_6	7642524	In contrast, the sphingosine  burst arose mainly from turnover of complex sphingolipids because no  incorporation of [ H]serine or  [ H]palmitate into sphingosine was detected;  sphingosine mass was not affected by beta-F-alanine or the serine  concentration; and, the burst could be followed by the release of  sphingosine and ceramide from complex sphingolipids (especially  sphingomyelin) in a process that was inhibited by NH Cl and  chloroquine.	transcription
61141	12	336082	5	NULL	NULL	0	NULL	statement 9	Process		is inhibited by					chloroquine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_32_18749_s_6	7642524	In contrast, the sphingosine  burst arose mainly from turnover of complex sphingolipids because no  incorporation of [ H]serine or  [ H]palmitate into sphingosine was detected;  sphingosine mass was not affected by beta-F-alanine or the serine  concentration; and, the burst could be followed by the release of  sphingosine and ceramide from complex sphingolipids (especially  sphingomyelin) in a process that was inhibited by NH Cl and  chloroquine.	transcription
61142	13	336082	5	NULL	NULL	0	NULL	statement 10	Process		is inhibited by					NH Cl	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_32_18749_s_6	7642524	In contrast, the sphingosine  burst arose mainly from turnover of complex sphingolipids because no  incorporation of [ H]serine or  [ H]palmitate into sphingosine was detected;  sphingosine mass was not affected by beta-F-alanine or the serine  concentration; and, the burst could be followed by the release of  sphingosine and ceramide from complex sphingolipids (especially  sphingomyelin) in a process that was inhibited by NH Cl and  chloroquine.	transcription
61143	14	336082	5	NULL	NULL	0	NULL	statement 10	Process		is inhibited by					chloroquine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_32_18749_s_6	7642524	In contrast, the sphingosine  burst arose mainly from turnover of complex sphingolipids because no  incorporation of [ H]serine or  [ H]palmitate into sphingosine was detected;  sphingosine mass was not affected by beta-F-alanine or the serine  concentration; and, the burst could be followed by the release of  sphingosine and ceramide from complex sphingolipids (especially  sphingomyelin) in a process that was inhibited by NH Cl and  chloroquine.	transcription
71927	1	336082	7	NULL	NULL	0	NULL	sphingosine	Chemical		released from					sphingomyelin	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_32_18749_s_6	7642524	In contrast, the sphingosine  burst arose mainly from turnover of complex sphingolipids because no  incorporation of [ H]serine or  [ H]palmitate into sphingosine was detected;  sphingosine mass was not affected by beta-F-alanine or the serine  concentration; and, the burst could be followed by the release of  sphingosine and ceramide from complex sphingolipids (especially  sphingomyelin) in a process that was inhibited by NH Cl and  chloroquine.	transcription
71928	2	336082	7	NULL	NULL	0	NULL	ceramide	Chemical		released from					sphingomyelin	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_32_18749_s_6	7642524	In contrast, the sphingosine  burst arose mainly from turnover of complex sphingolipids because no  incorporation of [ H]serine or  [ H]palmitate into sphingosine was detected;  sphingosine mass was not affected by beta-F-alanine or the serine  concentration; and, the burst could be followed by the release of  sphingosine and ceramide from complex sphingolipids (especially  sphingomyelin) in a process that was inhibited by NH Cl and  chloroquine.	transcription
71929	3	336082	7	NULL	NULL	0	NULL	NH Cl 	Chemical		inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_32_18749_s_6	7642524	In contrast, the sphingosine  burst arose mainly from turnover of complex sphingolipids because no  incorporation of [ H]serine or  [ H]palmitate into sphingosine was detected;  sphingosine mass was not affected by beta-F-alanine or the serine  concentration; and, the burst could be followed by the release of  sphingosine and ceramide from complex sphingolipids (especially  sphingomyelin) in a process that was inhibited by NH Cl and  chloroquine.	transcription
71930	4	336082	7	NULL	NULL	0	NULL	chloroquine	Chemical		inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_32_18749_s_6	7642524	In contrast, the sphingosine  burst arose mainly from turnover of complex sphingolipids because no  incorporation of [ H]serine or  [ H]palmitate into sphingosine was detected;  sphingosine mass was not affected by beta-F-alanine or the serine  concentration; and, the burst could be followed by the release of  sphingosine and ceramide from complex sphingolipids (especially  sphingomyelin) in a process that was inhibited by NH Cl and  chloroquine.	transcription
71931	5	336082	7	NULL	NULL	0	NULL	NH Cl 	Chemical		inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_32_18749_s_6	7642524	In contrast, the sphingosine  burst arose mainly from turnover of complex sphingolipids because no  incorporation of [ H]serine or  [ H]palmitate into sphingosine was detected;  sphingosine mass was not affected by beta-F-alanine or the serine  concentration; and, the burst could be followed by the release of  sphingosine and ceramide from complex sphingolipids (especially  sphingomyelin) in a process that was inhibited by NH Cl and  chloroquine.	transcription
71932	6	336082	7	NULL	NULL	0	NULL	chloroquine	Chemical		inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_32_18749_s_6	7642524	In contrast, the sphingosine  burst arose mainly from turnover of complex sphingolipids because no  incorporation of [ H]serine or  [ H]palmitate into sphingosine was detected;  sphingosine mass was not affected by beta-F-alanine or the serine  concentration; and, the burst could be followed by the release of  sphingosine and ceramide from complex sphingolipids (especially  sphingomyelin) in a process that was inhibited by NH Cl and  chloroquine.	transcription
71933	7	336082	7	NULL	NULL	0	NULL	sphingomyelin	Chemical		is a type of					complex sphingolipids	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_32_18749_s_6	7642524	In contrast, the sphingosine  burst arose mainly from turnover of complex sphingolipids because no  incorporation of [ H]serine or  [ H]palmitate into sphingosine was detected;  sphingosine mass was not affected by beta-F-alanine or the serine  concentration; and, the burst could be followed by the release of  sphingosine and ceramide from complex sphingolipids (especially  sphingomyelin) in a process that was inhibited by NH Cl and  chloroquine.	transcription
61144	1	336083	5	NULL	NULL	0	NULL	lung epithelia	OrganismPart		engage in					ceramide	Chemical	de novo synthesis of			NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_219	15772421	The new observations from these studies include the following:  i) that lung epithelia engage in high-level de novo ceramide synthesis using sphingoid bases;  ii) that D- erythro-[3-3H]sphingosine in lung cells is rapidly incorporated into ceramide, indicative of a robust  N-acyltransferase mechanism catalyzed by a ceramide synthase;  iii) that LASS5 is the predominant isoform conferring ceramide synthase activity that was developmentally regulated in the lung; and  iv) that PtdCho synthesis is dependently regulated with de novo ceramide synthesis.	transcription
61145	2	336083	5	NULL	NULL	0	NULL	statement 1	Process		uses					sphingoid bases	Chemical				NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_219	15772421	The new observations from these studies include the following:  i) that lung epithelia engage in high-level de novo ceramide synthesis using sphingoid bases;  ii) that D- erythro-[3-3H]sphingosine in lung cells is rapidly incorporated into ceramide, indicative of a robust  N-acyltransferase mechanism catalyzed by a ceramide synthase;  iii) that LASS5 is the predominant isoform conferring ceramide synthase activity that was developmentally regulated in the lung; and  iv) that PtdCho synthesis is dependently regulated with de novo ceramide synthesis.	transcription
61146	3	336083	5	NULL	NULL	0	NULL	D- erythro-[3-3H]sphingosine	Chemical		incorporated into		rapidly			ceramide	Chemical				NULL	lung cells	0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_219	15772421	The new observations from these studies include the following:  i) that lung epithelia engage in high-level de novo ceramide synthesis using sphingoid bases;  ii) that D- erythro-[3-3H]sphingosine in lung cells is rapidly incorporated into ceramide, indicative of a robust  N-acyltransferase mechanism catalyzed by a ceramide synthase;  iii) that LASS5 is the predominant isoform conferring ceramide synthase activity that was developmentally regulated in the lung; and  iv) that PtdCho synthesis is dependently regulated with de novo ceramide synthesis.	transcription
61147	4	336083	5	NULL	NULL	0	NULL	N-acyltransferase mechanism	Process		is catalyzed by					ceramide synthase	GP				NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_219	15772421	The new observations from these studies include the following:  i) that lung epithelia engage in high-level de novo ceramide synthesis using sphingoid bases;  ii) that D- erythro-[3-3H]sphingosine in lung cells is rapidly incorporated into ceramide, indicative of a robust  N-acyltransferase mechanism catalyzed by a ceramide synthase;  iii) that LASS5 is the predominant isoform conferring ceramide synthase activity that was developmentally regulated in the lung; and  iv) that PtdCho synthesis is dependently regulated with de novo ceramide synthesis.	transcription
61148	5	336083	5	NULL	NULL	0	NULL	statement 3	Process		indicates					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_219	15772421	The new observations from these studies include the following:  i) that lung epithelia engage in high-level de novo ceramide synthesis using sphingoid bases;  ii) that D- erythro-[3-3H]sphingosine in lung cells is rapidly incorporated into ceramide, indicative of a robust  N-acyltransferase mechanism catalyzed by a ceramide synthase;  iii) that LASS5 is the predominant isoform conferring ceramide synthase activity that was developmentally regulated in the lung; and  iv) that PtdCho synthesis is dependently regulated with de novo ceramide synthesis.	transcription
61149	6	336083	5	NULL	NULL	0	NULL	LASS5	GP		is an isoform of					ceramide synthase	GP				NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_219	15772421	The new observations from these studies include the following:  i) that lung epithelia engage in high-level de novo ceramide synthesis using sphingoid bases;  ii) that D- erythro-[3-3H]sphingosine in lung cells is rapidly incorporated into ceramide, indicative of a robust  N-acyltransferase mechanism catalyzed by a ceramide synthase;  iii) that LASS5 is the predominant isoform conferring ceramide synthase activity that was developmentally regulated in the lung; and  iv) that PtdCho synthesis is dependently regulated with de novo ceramide synthesis.	transcription
61150	7	336083	5	NULL	NULL	0	NULL	LASS5	GP		is developmentally regulated in					lung	OrganismPart				NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_219	15772421	The new observations from these studies include the following:  i) that lung epithelia engage in high-level de novo ceramide synthesis using sphingoid bases;  ii) that D- erythro-[3-3H]sphingosine in lung cells is rapidly incorporated into ceramide, indicative of a robust  N-acyltransferase mechanism catalyzed by a ceramide synthase;  iii) that LASS5 is the predominant isoform conferring ceramide synthase activity that was developmentally regulated in the lung; and  iv) that PtdCho synthesis is dependently regulated with de novo ceramide synthesis.	transcription
61151	8	336083	5	NULL	NULL	0	NULL	PtdCho	Chemical		is regulated in		dependently			ceramide	Chemical	de novo synthesis of			NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_219	15772421	The new observations from these studies include the following:  i) that lung epithelia engage in high-level de novo ceramide synthesis using sphingoid bases;  ii) that D- erythro-[3-3H]sphingosine in lung cells is rapidly incorporated into ceramide, indicative of a robust  N-acyltransferase mechanism catalyzed by a ceramide synthase;  iii) that LASS5 is the predominant isoform conferring ceramide synthase activity that was developmentally regulated in the lung; and  iv) that PtdCho synthesis is dependently regulated with de novo ceramide synthesis.	transcription
67559	1	336083	7	NULL	NULL	0	NULL	lung epithelia	Cell		engage in					de novo ceramide synthesis	Process	high-level of			NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_219	15772421	The new observations from these studies include the following:  i) that lung epithelia engage in high-level de novo ceramide synthesis using sphingoid bases;  ii) that D- erythro-[3-3H]sphingosine in lung cells is rapidly incorporated into ceramide, indicative of a robust  N-acyltransferase mechanism catalyzed by a ceramide synthase;  iii) that LASS5 is the predominant isoform conferring ceramide synthase activity that was developmentally regulated in the lung; and  iv) that PtdCho synthesis is dependently regulated with de novo ceramide synthesis.	transcription
67560	2	336083	7	NULL	NULL	0	NULL	statement 1	Process		use					sphingoid bases	Chemical				NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_219	15772421	The new observations from these studies include the following:  i) that lung epithelia engage in high-level de novo ceramide synthesis using sphingoid bases;  ii) that D- erythro-[3-3H]sphingosine in lung cells is rapidly incorporated into ceramide, indicative of a robust  N-acyltransferase mechanism catalyzed by a ceramide synthase;  iii) that LASS5 is the predominant isoform conferring ceramide synthase activity that was developmentally regulated in the lung; and  iv) that PtdCho synthesis is dependently regulated with de novo ceramide synthesis.	transcription
67561	3	336083	7	NULL	NULL	0	NULL	D- erythro-[3-3H]sphingosine	Chemical	lung cells	incorporated into					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_219	15772421	The new observations from these studies include the following:  i) that lung epithelia engage in high-level de novo ceramide synthesis using sphingoid bases;  ii) that D- erythro-[3-3H]sphingosine in lung cells is rapidly incorporated into ceramide, indicative of a robust  N-acyltransferase mechanism catalyzed by a ceramide synthase;  iii) that LASS5 is the predominant isoform conferring ceramide synthase activity that was developmentally regulated in the lung; and  iv) that PtdCho synthesis is dependently regulated with de novo ceramide synthesis.	transcription
67562	4	336083	7	NULL	NULL	0	NULL	statement 3	Process		indicative of					N-acyltransferase mechanism	Process				NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_219	15772421	The new observations from these studies include the following:  i) that lung epithelia engage in high-level de novo ceramide synthesis using sphingoid bases;  ii) that D- erythro-[3-3H]sphingosine in lung cells is rapidly incorporated into ceramide, indicative of a robust  N-acyltransferase mechanism catalyzed by a ceramide synthase;  iii) that LASS5 is the predominant isoform conferring ceramide synthase activity that was developmentally regulated in the lung; and  iv) that PtdCho synthesis is dependently regulated with de novo ceramide synthesis.	transcription
67563	5	336083	7	NULL	NULL	0	NULL	statement 4	Process		catalyzed by					ceramide synthase	GP				NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_219	15772421	The new observations from these studies include the following:  i) that lung epithelia engage in high-level de novo ceramide synthesis using sphingoid bases;  ii) that D- erythro-[3-3H]sphingosine in lung cells is rapidly incorporated into ceramide, indicative of a robust  N-acyltransferase mechanism catalyzed by a ceramide synthase;  iii) that LASS5 is the predominant isoform conferring ceramide synthase activity that was developmentally regulated in the lung; and  iv) that PtdCho synthesis is dependently regulated with de novo ceramide synthesis.	transcription
67564	6	336083	7	NULL	NULL	NULL	NULL	LASS5	GP	predominant isoform	confer					ceramide synthase activity	Process				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_219	15772421	The new observations from these studies include the following:  i) that lung epithelia engage in high-level de novo ceramide synthesis using sphingoid bases;  ii) that D- erythro-[3-3H]sphingosine in lung cells is rapidly incorporated into ceramide, indicative of a robust  N-acyltransferase mechanism catalyzed by a ceramide synthase;  iii) that LASS5 is the predominant isoform conferring ceramide synthase activity that was developmentally regulated in the lung; and  iv) that PtdCho synthesis is dependently regulated with de novo ceramide synthesis.	transcription
67565	7	336083	7	NULL	NULL	NULL	NULL	 ceramide synthase activity	Process		regulated in the 		developmentally			lung	OrganismPart				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_219	15772421	The new observations from these studies include the following:  i) that lung epithelia engage in high-level de novo ceramide synthesis using sphingoid bases;  ii) that D- erythro-[3-3H]sphingosine in lung cells is rapidly incorporated into ceramide, indicative of a robust  N-acyltransferase mechanism catalyzed by a ceramide synthase;  iii) that LASS5 is the predominant isoform conferring ceramide synthase activity that was developmentally regulated in the lung; and  iv) that PtdCho synthesis is dependently regulated with de novo ceramide synthesis.	transcription
67566	8	336083	7	NULL	NULL	0	NULL	PtdCho synthesis	Process		regulated with		dependently			de novo ceramide synthesis	Process				NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_219	15772421	The new observations from these studies include the following:  i) that lung epithelia engage in high-level de novo ceramide synthesis using sphingoid bases;  ii) that D- erythro-[3-3H]sphingosine in lung cells is rapidly incorporated into ceramide, indicative of a robust  N-acyltransferase mechanism catalyzed by a ceramide synthase;  iii) that LASS5 is the predominant isoform conferring ceramide synthase activity that was developmentally regulated in the lung; and  iv) that PtdCho synthesis is dependently regulated with de novo ceramide synthesis.	transcription
61152	1	336084	5	NULL	NULL	0	NULL	ceramidase	GP	activated	removes					ceramide	Chemical	excess			NULL	human umbilical vein endothelial cells	0	NULL	NULL	NULL	gw70_jbiolchem_278_29_26992_s_26	12721293	Also,  removal of excess ceramide in human umbilical vein endothelial cells by  activating ceramidase prevents TNF-alpha-induced cell death and the  resulting accumulation of sphingosine and sphingosine phosphate induces the  expression of the adhesion molecules E-selectin and vascular cell adhesion  molecule-1 ( ).	transcription
61153	2	336084	5	NULL	NULL	0	NULL	cell death	Process		is induced by					TNF-alpha	GP				NULL	human umbilical vein endothelial cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26992_s_26	12721293	Also,  removal of excess ceramide in human umbilical vein endothelial cells by  activating ceramidase prevents TNF-alpha-induced cell death and the  resulting accumulation of sphingosine and sphingosine phosphate induces the  expression of the adhesion molecules E-selectin and vascular cell adhesion  molecule-1 ( ).	transcription
61154	3	336084	5	NULL	NULL	0	NULL	statement 1	Process		prevents					statement 2	Process				NULL	human umbilical vein endothelial cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26992_s_26	12721293	Also,  removal of excess ceramide in human umbilical vein endothelial cells by  activating ceramidase prevents TNF-alpha-induced cell death and the  resulting accumulation of sphingosine and sphingosine phosphate induces the  expression of the adhesion molecules E-selectin and vascular cell adhesion  molecule-1 ( ).	transcription
61157	4	336084	5	NULL	NULL	0	NULL	statement 3	Process		results in					sphingosine	Process	accumulation of			NULL	human umbilical vein endothelial cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26992_s_26	12721293	Also,  removal of excess ceramide in human umbilical vein endothelial cells by  activating ceramidase prevents TNF-alpha-induced cell death and the  resulting accumulation of sphingosine and sphingosine phosphate induces the  expression of the adhesion molecules E-selectin and vascular cell adhesion  molecule-1 ( ).	transcription
61158	5	336084	5	NULL	NULL	0	NULL	statement 3	Process		results in					sphingosine phosphate	Chemical	accumulation of			NULL	human umbilical vein endothelial cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26992_s_26	12721293	Also,  removal of excess ceramide in human umbilical vein endothelial cells by  activating ceramidase prevents TNF-alpha-induced cell death and the  resulting accumulation of sphingosine and sphingosine phosphate induces the  expression of the adhesion molecules E-selectin and vascular cell adhesion  molecule-1 ( ).	transcription
61159	6	336084	5	NULL	NULL	0	NULL	statement 4	Process		induce					E-selectin	GP	expression of			NULL	human umbilical vein endothelial cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26992_s_26	12721293	Also,  removal of excess ceramide in human umbilical vein endothelial cells by  activating ceramidase prevents TNF-alpha-induced cell death and the  resulting accumulation of sphingosine and sphingosine phosphate induces the  expression of the adhesion molecules E-selectin and vascular cell adhesion  molecule-1 ( ).	transcription
61160	7	336084	5	NULL	NULL	0	NULL	statement 4	Process		induce					vascular cell adhesion molecule-1 	GP	expression of			NULL	human umbilical vein endothelial cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26992_s_26	12721293	Also,  removal of excess ceramide in human umbilical vein endothelial cells by  activating ceramidase prevents TNF-alpha-induced cell death and the  resulting accumulation of sphingosine and sphingosine phosphate induces the  expression of the adhesion molecules E-selectin and vascular cell adhesion  molecule-1 ( ).	transcription
61161	8	336084	5	NULL	NULL	0	NULL	statement 5	Process		induce					E-selectin	GP	expression of			NULL	human umbilical vein endothelial cells	NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26992_s_26	12721293	Also,  removal of excess ceramide in human umbilical vein endothelial cells by  activating ceramidase prevents TNF-alpha-induced cell death and the  resulting accumulation of sphingosine and sphingosine phosphate induces the  expression of the adhesion molecules E-selectin and vascular cell adhesion  molecule-1 ( ).	transcription
61162	9	336084	5	NULL	NULL	0	NULL	statement 4	Process		induce					vascular cell adhesion molecule-1 	GP	expression of			NULL	human umbilical vein endothelial cells	0	NULL	NULL	NULL	gw70_jbiolchem_278_29_26992_s_26	12721293	Also,  removal of excess ceramide in human umbilical vein endothelial cells by  activating ceramidase prevents TNF-alpha-induced cell death and the  resulting accumulation of sphingosine and sphingosine phosphate induces the  expression of the adhesion molecules E-selectin and vascular cell adhesion  molecule-1 ( ).	transcription
61163	10	336084	5	NULL	NULL	0	NULL	E-selectin	GP		is a type of					adhesion molecule	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_29_26992_s_26	12721293	Also,  removal of excess ceramide in human umbilical vein endothelial cells by  activating ceramidase prevents TNF-alpha-induced cell death and the  resulting accumulation of sphingosine and sphingosine phosphate induces the  expression of the adhesion molecules E-selectin and vascular cell adhesion  molecule-1 ( ).	transcription
61164	11	336084	5	NULL	NULL	0	NULL	vascular cell adhesion molecule-1	GP		is a type of					adhesion molecule	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_29_26992_s_26	12721293	Also,  removal of excess ceramide in human umbilical vein endothelial cells by  activating ceramidase prevents TNF-alpha-induced cell death and the  resulting accumulation of sphingosine and sphingosine phosphate induces the  expression of the adhesion molecules E-selectin and vascular cell adhesion  molecule-1 ( ).	transcription
67567	1	336084	7	NULL	NULL	0	NULL	ceramidase	GP	activating	remove					ceramide	Chemical	excess of			NULL	human umbilical vein endothelial cells	0	NULL	NULL	NULL	gw70_jbiolchem_278_29_26992_s_26	12721293	Also,  removal of excess ceramide in human umbilical vein endothelial cells by  activating ceramidase prevents TNF-alpha-induced cell death and the  resulting accumulation of sphingosine and sphingosine phosphate induces the  expression of the adhesion molecules E-selectin and vascular cell adhesion  molecule-1 ( ).	transcription
67568	2	336084	7	NULL	NULL	0	NULL	TNF-alpha	GP		induce					cell death	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_29_26992_s_26	12721293	Also,  removal of excess ceramide in human umbilical vein endothelial cells by  activating ceramidase prevents TNF-alpha-induced cell death and the  resulting accumulation of sphingosine and sphingosine phosphate induces the  expression of the adhesion molecules E-selectin and vascular cell adhesion  molecule-1 ( ).	transcription
67569	3	336084	7	NULL	NULL	0	NULL	statement 1	Process		prevents					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_29_26992_s_26	12721293	Also,  removal of excess ceramide in human umbilical vein endothelial cells by  activating ceramidase prevents TNF-alpha-induced cell death and the  resulting accumulation of sphingosine and sphingosine phosphate induces the  expression of the adhesion molecules E-selectin and vascular cell adhesion  molecule-1 ( ).	transcription
67570	4	336084	7	NULL	NULL	0	NULL	statement 3	Process		result in					sphingosine	Chemical	accumulation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_29_26992_s_26	12721293	Also,  removal of excess ceramide in human umbilical vein endothelial cells by  activating ceramidase prevents TNF-alpha-induced cell death and the  resulting accumulation of sphingosine and sphingosine phosphate induces the  expression of the adhesion molecules E-selectin and vascular cell adhesion  molecule-1 ( ).	transcription
67571	5	336084	7	NULL	NULL	0	NULL	statement 3	Process		result in					sphingosine phosphate	Chemical	accumulation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_29_26992_s_26	12721293	Also,  removal of excess ceramide in human umbilical vein endothelial cells by  activating ceramidase prevents TNF-alpha-induced cell death and the  resulting accumulation of sphingosine and sphingosine phosphate induces the  expression of the adhesion molecules E-selectin and vascular cell adhesion  molecule-1 ( ).	transcription
67572	6	336084	7	NULL	NULL	NULL	NULL	sphingosine	Chemical		induce					E-selectin	Chemical	expression of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26992_s_26	12721293	Also,  removal of excess ceramide in human umbilical vein endothelial cells by  activating ceramidase prevents TNF-alpha-induced cell death and the  resulting accumulation of sphingosine and sphingosine phosphate induces the  expression of the adhesion molecules E-selectin and vascular cell adhesion  molecule-1 ( ).	transcription
67573	7	336084	7	NULL	NULL	NULL	NULL	sphingosine phosphate	Chemical		induce					E-selectin	Chemical	expression of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26992_s_26	12721293	Also,  removal of excess ceramide in human umbilical vein endothelial cells by  activating ceramidase prevents TNF-alpha-induced cell death and the  resulting accumulation of sphingosine and sphingosine phosphate induces the  expression of the adhesion molecules E-selectin and vascular cell adhesion  molecule-1 ( ).	transcription
67574	8	336084	7	NULL	NULL	0	NULL	sphingosine	Chemical		induce					vascular cell adhesion molecule-1	Chemical	expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_29_26992_s_26	12721293	Also,  removal of excess ceramide in human umbilical vein endothelial cells by  activating ceramidase prevents TNF-alpha-induced cell death and the  resulting accumulation of sphingosine and sphingosine phosphate induces the  expression of the adhesion molecules E-selectin and vascular cell adhesion  molecule-1 ( ).	transcription
67575	9	336084	7	NULL	NULL	0	NULL	sphingosine phosphate	Chemical		induce					vascular cell adhesion molecule-1	Chemical	expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_29_26992_s_26	12721293	Also,  removal of excess ceramide in human umbilical vein endothelial cells by  activating ceramidase prevents TNF-alpha-induced cell death and the  resulting accumulation of sphingosine and sphingosine phosphate induces the  expression of the adhesion molecules E-selectin and vascular cell adhesion  molecule-1 ( ).	transcription
67576	10	336084	7	NULL	NULL	NULL	NULL	E-selectin	Chemical		is a type of					adhesion molecule	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_29_26992_s_26	12721293	Also,  removal of excess ceramide in human umbilical vein endothelial cells by  activating ceramidase prevents TNF-alpha-induced cell death and the  resulting accumulation of sphingosine and sphingosine phosphate induces the  expression of the adhesion molecules E-selectin and vascular cell adhesion  molecule-1 ( ).	transcription
67577	11	336084	7	NULL	NULL	0	NULL	vascular cell adhesion molecule-1	Chemical		is a type of					adhesion molecule	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_29_26992_s_26	12721293	Also,  removal of excess ceramide in human umbilical vein endothelial cells by  activating ceramidase prevents TNF-alpha-induced cell death and the  resulting accumulation of sphingosine and sphingosine phosphate induces the  expression of the adhesion molecules E-selectin and vascular cell adhesion  molecule-1 ( ).	transcription
61165	1	336085	5	NULL	NULL	0	NULL	sphingosine	GP		activates					executioner caspases	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_92	10747891	Sphingosine Induces Apoptosis by Activation of Executioner Caspases in a Bcl-xL-inhibitable Fashion-- Because current evidence suggests that ceramide functions proximal to the executioner caspases ( 15,  37), we examined whether addition of sphingosine resulted in activation of caspase-3 and -7, which drive the effector phase of apoptosis.	transcription
61166	2	336085	5	NULL	NULL	0	NULL	statement 1	Process		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_92	10747891	Sphingosine Induces Apoptosis by Activation of Executioner Caspases in a Bcl-xL-inhibitable Fashion-- Because current evidence suggests that ceramide functions proximal to the executioner caspases ( 15,  37), we examined whether addition of sphingosine resulted in activation of caspase-3 and -7, which drive the effector phase of apoptosis.	transcription
61167	3	336085	5	NULL	NULL	0	NULL	statement 2	Process		is inhibited by					Bcl-xL	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_92	10747891	Sphingosine Induces Apoptosis by Activation of Executioner Caspases in a Bcl-xL-inhibitable Fashion-- Because current evidence suggests that ceramide functions proximal to the executioner caspases ( 15,  37), we examined whether addition of sphingosine resulted in activation of caspase-3 and -7, which drive the effector phase of apoptosis.	transcription
61168	4	336085	5	NULL	NULL	0	NULL	ceramide	Chemical	functional	is proximal to					executioner caspases	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_92	10747891	Sphingosine Induces Apoptosis by Activation of Executioner Caspases in a Bcl-xL-inhibitable Fashion-- Because current evidence suggests that ceramide functions proximal to the executioner caspases ( 15,  37), we examined whether addition of sphingosine resulted in activation of caspase-3 and -7, which drive the effector phase of apoptosis.	transcription
61169	5	336085	5	NULL	NULL	0	NULL	caspase-3	GP	activation of	drives					apoptosis	Process	effector phase of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_92	10747891	Sphingosine Induces Apoptosis by Activation of Executioner Caspases in a Bcl-xL-inhibitable Fashion-- Because current evidence suggests that ceramide functions proximal to the executioner caspases ( 15,  37), we examined whether addition of sphingosine resulted in activation of caspase-3 and -7, which drive the effector phase of apoptosis.	transcription
61170	6	336085	5	NULL	NULL	0	NULL	caspase-7	GP	activation of	drives					apoptosis	Process	effector phase of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_92	10747891	Sphingosine Induces Apoptosis by Activation of Executioner Caspases in a Bcl-xL-inhibitable Fashion-- Because current evidence suggests that ceramide functions proximal to the executioner caspases ( 15,  37), we examined whether addition of sphingosine resulted in activation of caspase-3 and -7, which drive the effector phase of apoptosis.	transcription
61171	7	336085	5	NULL	NULL	0	NULL	sphingosine	Chemical	addition of	activates		potentially			statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_92	10747891	Sphingosine Induces Apoptosis by Activation of Executioner Caspases in a Bcl-xL-inhibitable Fashion-- Because current evidence suggests that ceramide functions proximal to the executioner caspases ( 15,  37), we examined whether addition of sphingosine resulted in activation of caspase-3 and -7, which drive the effector phase of apoptosis.	transcription
61172	8	336085	5	NULL	NULL	0	NULL	sphingosine	Chemical	addition of	activates		potentially			statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_92	10747891	Sphingosine Induces Apoptosis by Activation of Executioner Caspases in a Bcl-xL-inhibitable Fashion-- Because current evidence suggests that ceramide functions proximal to the executioner caspases ( 15,  37), we examined whether addition of sphingosine resulted in activation of caspase-3 and -7, which drive the effector phase of apoptosis.	transcription
67578	1	336085	7	NULL	NULL	0	NULL	Sphingosine	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_92	10747891	Sphingosine Induces Apoptosis by Activation of Executioner Caspases in a Bcl-xL-inhibitable Fashion-- Because current evidence suggests that ceramide functions proximal to the executioner caspases ( 15,  37), we examined whether addition of sphingosine resulted in activation of caspase-3 and -7, which drive the effector phase of apoptosis.	transcription
67579	2	336085	7	NULL	NULL	0	NULL	statement 1	Process		occur by					Executioner Caspases	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_92	10747891	Sphingosine Induces Apoptosis by Activation of Executioner Caspases in a Bcl-xL-inhibitable Fashion-- Because current evidence suggests that ceramide functions proximal to the executioner caspases ( 15,  37), we examined whether addition of sphingosine resulted in activation of caspase-3 and -7, which drive the effector phase of apoptosis.	transcription
67580	3	336085	7	NULL	NULL	0	NULL	statement 2	Process		occur in a					Bcl-xL-inhibitable Fashion	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_92	10747891	Sphingosine Induces Apoptosis by Activation of Executioner Caspases in a Bcl-xL-inhibitable Fashion-- Because current evidence suggests that ceramide functions proximal to the executioner caspases ( 15,  37), we examined whether addition of sphingosine resulted in activation of caspase-3 and -7, which drive the effector phase of apoptosis.	transcription
67581	4	336085	7	NULL	NULL	0	NULL	ceramide	Chemical		functions					Executioner Caspases	GP	proximal to			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_92	10747891	Sphingosine Induces Apoptosis by Activation of Executioner Caspases in a Bcl-xL-inhibitable Fashion-- Because current evidence suggests that ceramide functions proximal to the executioner caspases ( 15,  37), we examined whether addition of sphingosine resulted in activation of caspase-3 and -7, which drive the effector phase of apoptosis.	transcription
67582	5	336085	7	NULL	NULL	0	NULL	caspase-3	GP		drive					apoptosis	Process	effector phase of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_92	10747891	Sphingosine Induces Apoptosis by Activation of Executioner Caspases in a Bcl-xL-inhibitable Fashion-- Because current evidence suggests that ceramide functions proximal to the executioner caspases ( 15,  37), we examined whether addition of sphingosine resulted in activation of caspase-3 and -7, which drive the effector phase of apoptosis.	transcription
67583	6	336085	7	NULL	NULL	0	NULL	caspase-7	GP		drive					apoptosis	Process	effector phase of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_92	10747891	Sphingosine Induces Apoptosis by Activation of Executioner Caspases in a Bcl-xL-inhibitable Fashion-- Because current evidence suggests that ceramide functions proximal to the executioner caspases ( 15,  37), we examined whether addition of sphingosine resulted in activation of caspase-3 and -7, which drive the effector phase of apoptosis.	transcription
61173	1	336087	5	NULL	NULL	0	NULL	3T3-L1 adipocytes	Cell		treated with					short-chain ceramide	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
61174	2	336087	5	NULL	NULL	0	NULL	3T3-L1 adipocytes	Cell		treated with					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
61175	3	336087	5	NULL	NULL	0	NULL	3T3-L1 adipocytes	Cell		treated with					S1P	Chemical				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
61176	4	336087	5	NULL	NULL	0	NULL	statement 1	Process		induce					PAI-1	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
61177	5	336087	5	NULL	NULL	0	NULL	statement 2	Process		induce					PAI-1	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
61178	6	336087	5	NULL	NULL	0	NULL	statement 3	Process		induce					PAI-1	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
61179	7	336087	5	NULL	NULL	0	NULL	PAI-1	GP		is a type of					prothrombotic molecule	GP				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
61180	8	336087	5	NULL	NULL	0	NULL	statement 1	Process		induce					TNF-alpha	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
61181	9	336087	5	NULL	NULL	0	NULL	statement 2	Process		induce					TNF-alpha	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
61182	10	336087	5	NULL	NULL	0	NULL	statement 3	Process		induce					TNF-alpha	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
61183	11	336087	5	NULL	NULL	0	NULL	statement 1	Process		induce					IL-6	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
61184	12	336087	5	NULL	NULL	0	NULL	statement 2	Process		induce					IL-6	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
61185	13	336087	5	NULL	NULL	0	NULL	statement 3	Process		induce					IL-6	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
61186	14	336087	5	NULL	NULL	0	NULL	statement 1	Process		induce					MCP-1	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
61187	15	336087	5	NULL	NULL	0	NULL	statement 2	Process		induce					MCP-1	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
61188	16	336087	5	NULL	NULL	0	NULL	statement 3	Process		induce					MCP-1	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
61189	17	336087	5	NULL	NULL	0	NULL	statement 1	Process		induce					KC	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
61190	18	336087	5	NULL	NULL	0	NULL	statement 2	Process		induce					KC	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
61191	19	336087	5	NULL	NULL	0	NULL	statement 3	Process		induce					KC	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
61192	20	336087	5	NULL	NULL	0	NULL	TNF-alpha	GP		is a type of					proinflammatory molecule	GP				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
61193	21	336087	5	NULL	NULL	0	NULL	IL-6	GP		is a type of					proinflammatory molecule	GP				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
61194	22	336087	5	NULL	NULL	0	NULL	MCP-1	GP		is a type of					proinflammatory molecule	GP				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
61195	23	336087	5	NULL	NULL	0	NULL	KC	GP		is a type of					proinflammatory molecule	GP				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
67584	1	336087	7	NULL	NULL	NULL	NULL	short-chain ceramide	Chemical		induce					PAI-1	GP	expression of			NULL	 3T3-L1 adipocytes	NULL	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
67585	2	336087	7	NULL	NULL	NULL	NULL	sphingosine	Chemical		induce					PAI-1	GP	expression of			NULL	 3T3-L1 adipocytes	NULL	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
67586	3	336087	7	NULL	NULL	NULL	NULL	 S1P	Chemical		induce					PAI-1	GP	expression of			NULL	 3T3-L1 adipocytes	NULL	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
67587	4	336087	7	NULL	NULL	0	NULL	PAI-1	GP		is a type of					prothrombotic molecule	GP				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
67588	5	336087	7	NULL	NULL	0	NULL	short-chain ceramide	Chemical		induce					TNF-alpha	GP	expression of			NULL	3T3-L1 adipocytes	0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
67589	6	336087	7	NULL	NULL	NULL	NULL	sphingosine	Chemical		induce					TNF-alpha	GP	expression of			NULL	3T3-L1 adipocytes	NULL	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
67590	7	336087	7	NULL	NULL	NULL	NULL	S1P	Chemical		induce					TNF-alpha	GP	expression of			NULL	3T3-L1 adipocytes	NULL	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
67591	8	336087	7	NULL	NULL	0	NULL	 short-chain ceramide	Chemical		induce					IL-6	GP	expression of			NULL	3T3-L1 adipocytes	0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
67592	9	336087	7	NULL	NULL	0	NULL	sphingosine	Chemical		induce					IL-6	GP	expression of			NULL	3T3-L1 adipocytes	0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
67593	10	336087	7	NULL	NULL	0	NULL	S1P	Chemical		induce					IL-6	GP	expression of			NULL	3T3-L1 adipocytes	0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
67594	11	336087	7	NULL	NULL	NULL	NULL	short-chain ceramide	Chemical		induce					MCP-1	GP	expression of			NULL	3T3-L1 adipocytes	NULL	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
67595	12	336087	7	NULL	NULL	NULL	NULL	sphingosine	Chemical		induce					MCP-1	GP	expression of			NULL	3T3-L1 adipocytes	NULL	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
67596	13	336087	7	NULL	NULL	NULL	NULL	S1P	Chemical		induce					MCP-1	GP	expression of			NULL	3T3-L1 adipocytes	NULL	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
67597	14	336087	7	NULL	NULL	0	NULL	short-chain ceramide	Chemical		induce					KC	GP	expression of			NULL	3T3-L1 adipocytes	0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
67598	15	336087	7	NULL	NULL	0	NULL	sphingosine	Chemical		induce					KC	GP	expression of			NULL	3T3-L1 adipocytes	0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
67599	16	336087	7	NULL	NULL	0	NULL	 S1P	Chemical		induce					KC	GP	expression of			NULL	3T3-L1 adipocytes	0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
67600	17	336087	7	NULL	NULL	0	NULL	TNF-alpha	GP		is a type of					proinflammatory molecule	GP				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
67601	18	336087	7	NULL	NULL	0	NULL	IL-6	GP		is a type of					proinflammatory molecule	GP				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
67602	19	336087	7	NULL	NULL	0	NULL	MCP-1	GP		is a type of					proinflammatory molecule	GP				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
67603	20	336087	7	NULL	NULL	0	NULL	KC	GP		is a type of					proinflammatory molecule	GP				NULL		0	NULL	NULL	NULL	gw70_diabetes_55_9_2579_s_191	16936207	We demonstrate that treatment of 3T3-L1 adipocytes with short-chain ceramide, sphingosine, or S1P induced the expression of the prothrombotic molecule PAI-1 and the expression of the proinflammatory molecules, TNF-alpha, IL-6, MCP-1, and KC ( Fig. 5) to various extents.	transcription
61196	1	336088	5	NULL	NULL	0	NULL	ceramide	Chemical		is converted to					sphingosine	Chemical				NULL	lysosome	0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_11	15774472	To determine the contribution of either sphingolipid in FFA-dependent inhibition of insulin action, we generated C2C12 myotubes that constitutively overexpress  acid  ceramidase (AC), an enzyme that catalyzes the lysosomal conversion of ceramide to sphingosine.	transcription
61197	2	336088	5	NULL	NULL	0	NULL	AC	GP		catalyzes					statement 1	Process				NULL	lysosome	0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_11	15774472	To determine the contribution of either sphingolipid in FFA-dependent inhibition of insulin action, we generated C2C12 myotubes that constitutively overexpress  acid  ceramidase (AC), an enzyme that catalyzes the lysosomal conversion of ceramide to sphingosine.	transcription
61198	3	336088	5	NULL	NULL	0	NULL	AC	GP		is					acid ceramidase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_11	15774472	To determine the contribution of either sphingolipid in FFA-dependent inhibition of insulin action, we generated C2C12 myotubes that constitutively overexpress  acid  ceramidase (AC), an enzyme that catalyzes the lysosomal conversion of ceramide to sphingosine.	transcription
61199	4	336088	5	NULL	NULL	0	NULL	insulin	GP	inhibition of;;action of	is dependent on					FFA	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_11	15774472	To determine the contribution of either sphingolipid in FFA-dependent inhibition of insulin action, we generated C2C12 myotubes that constitutively overexpress  acid  ceramidase (AC), an enzyme that catalyzes the lysosomal conversion of ceramide to sphingosine.	transcription
61200	5	336088	5	NULL	NULL	0	NULL	sphingolipid	Chemical		contribute to		potentially			statement 4					NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_11	15774472	To determine the contribution of either sphingolipid in FFA-dependent inhibition of insulin action, we generated C2C12 myotubes that constitutively overexpress  acid  ceramidase (AC), an enzyme that catalyzes the lysosomal conversion of ceramide to sphingosine.	transcription
67604	1	336088	7	NULL	NULL	0	NULL	 ceramide	Chemical		converted to					sphingosine	Chemical				NULL	lysosomes	0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_11	15774472	To determine the contribution of either sphingolipid in FFA-dependent inhibition of insulin action, we generated C2C12 myotubes that constitutively overexpress  acid  ceramidase (AC), an enzyme that catalyzes the lysosomal conversion of ceramide to sphingosine.	transcription
67605	2	336088	7	NULL	NULL	0	NULL	AC	GP		catalyze					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_11	15774472	To determine the contribution of either sphingolipid in FFA-dependent inhibition of insulin action, we generated C2C12 myotubes that constitutively overexpress  acid  ceramidase (AC), an enzyme that catalyzes the lysosomal conversion of ceramide to sphingosine.	transcription
67606	3	336088	7	NULL	NULL	0	NULL	AC	GP		is					acid ceramidase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_11	15774472	To determine the contribution of either sphingolipid in FFA-dependent inhibition of insulin action, we generated C2C12 myotubes that constitutively overexpress  acid  ceramidase (AC), an enzyme that catalyzes the lysosomal conversion of ceramide to sphingosine.	transcription
61201	1	336089	5	NULL	NULL	0	NULL	palmitate	Chemical		inhibits					Akt/PKB	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_76	15774472	Under conditions where palmitate inhibits Akt/PKB, it induces the accumulation of both ceramide and sphingosine ( Fig. 1), two lipid metabolites shown previously to inhibit insulin-stimulated glucose transport ( ,   -  ).	transcription
61202	2	336089	5	NULL	NULL	0	NULL	statement 1	Process		induce					ceramide	Chemical	accumulation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_76	15774472	Under conditions where palmitate inhibits Akt/PKB, it induces the accumulation of both ceramide and sphingosine ( Fig. 1), two lipid metabolites shown previously to inhibit insulin-stimulated glucose transport ( ,   -  ).	transcription
61203	3	336089	5	NULL	NULL	0	NULL	statement 1	Process		induce					sphingosine	Chemical	accumulation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_76	15774472	Under conditions where palmitate inhibits Akt/PKB, it induces the accumulation of both ceramide and sphingosine ( Fig. 1), two lipid metabolites shown previously to inhibit insulin-stimulated glucose transport ( ,   -  ).	transcription
61204	4	336089	5	NULL	NULL	0	NULL	ceramide	Chemical		is a metabolite of					lipid	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_76	15774472	Under conditions where palmitate inhibits Akt/PKB, it induces the accumulation of both ceramide and sphingosine ( Fig. 1), two lipid metabolites shown previously to inhibit insulin-stimulated glucose transport ( ,   -  ).	transcription
61205	5	336089	5	NULL	NULL	0	NULL	sphingosine	Chemical		is a metabolite of					lipid	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_76	15774472	Under conditions where palmitate inhibits Akt/PKB, it induces the accumulation of both ceramide and sphingosine ( Fig. 1), two lipid metabolites shown previously to inhibit insulin-stimulated glucose transport ( ,   -  ).	transcription
61206	6	336089	5	NULL	NULL	0	NULL	glucose	Chemical	transport of	is stimulated by					insulin	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_76	15774472	Under conditions where palmitate inhibits Akt/PKB, it induces the accumulation of both ceramide and sphingosine ( Fig. 1), two lipid metabolites shown previously to inhibit insulin-stimulated glucose transport ( ,   -  ).	transcription
61207	7	336089	5	NULL	NULL	0	NULL	ceramide	Chemical		inhibits					statement 6	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_76	15774472	Under conditions where palmitate inhibits Akt/PKB, it induces the accumulation of both ceramide and sphingosine ( Fig. 1), two lipid metabolites shown previously to inhibit insulin-stimulated glucose transport ( ,   -  ).	transcription
61208	8	336089	5	NULL	NULL	0	NULL	sphingosine	Chemical		inhibits					statement 6	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_76	15774472	Under conditions where palmitate inhibits Akt/PKB, it induces the accumulation of both ceramide and sphingosine ( Fig. 1), two lipid metabolites shown previously to inhibit insulin-stimulated glucose transport ( ,   -  ).	transcription
67607	1	336089	7	NULL	NULL	0	NULL	 palmitate	Chemical		inhibits					Akt/PKB	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_76	15774472	Under conditions where palmitate inhibits Akt/PKB, it induces the accumulation of both ceramide and sphingosine ( Fig. 1), two lipid metabolites shown previously to inhibit insulin-stimulated glucose transport ( ,   -  ).	transcription
67608	2	336089	7	NULL	NULL	0	NULL	statement 1	Process		induce					ceramide	Chemical	accumulation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_76	15774472	Under conditions where palmitate inhibits Akt/PKB, it induces the accumulation of both ceramide and sphingosine ( Fig. 1), two lipid metabolites shown previously to inhibit insulin-stimulated glucose transport ( ,   -  ).	transcription
67609	3	336089	7	NULL	NULL	0	NULL	statement 1	Process		induce					sphingosine	Chemical	accumulation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_76	15774472	Under conditions where palmitate inhibits Akt/PKB, it induces the accumulation of both ceramide and sphingosine ( Fig. 1), two lipid metabolites shown previously to inhibit insulin-stimulated glucose transport ( ,   -  ).	transcription
67610	4	336089	7	NULL	NULL	0	NULL	insulin	GP		stimulate					glucose transport	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_76	15774472	Under conditions where palmitate inhibits Akt/PKB, it induces the accumulation of both ceramide and sphingosine ( Fig. 1), two lipid metabolites shown previously to inhibit insulin-stimulated glucose transport ( ,   -  ).	transcription
67611	5	336089	7	NULL	NULL	NULL	NULL	ceramide	Chemical		inhibit					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_76	15774472	Under conditions where palmitate inhibits Akt/PKB, it induces the accumulation of both ceramide and sphingosine ( Fig. 1), two lipid metabolites shown previously to inhibit insulin-stimulated glucose transport ( ,   -  ).	transcription
67612	6	336089	7	NULL	NULL	0	NULL	sphingosine	Chemical		inhibit					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_76	15774472	Under conditions where palmitate inhibits Akt/PKB, it induces the accumulation of both ceramide and sphingosine ( Fig. 1), two lipid metabolites shown previously to inhibit insulin-stimulated glucose transport ( ,   -  ).	transcription
67613	7	336089	7	NULL	NULL	0	NULL	ceramide	Chemical		is a type of					lipid metabolite	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_76	15774472	Under conditions where palmitate inhibits Akt/PKB, it induces the accumulation of both ceramide and sphingosine ( Fig. 1), two lipid metabolites shown previously to inhibit insulin-stimulated glucose transport ( ,   -  ).	transcription
67614	8	336089	7	NULL	NULL	0	NULL	sphingosine	Chemical		is a type of					lipid metabolite	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20148_s_76	15774472	Under conditions where palmitate inhibits Akt/PKB, it induces the accumulation of both ceramide and sphingosine ( Fig. 1), two lipid metabolites shown previously to inhibit insulin-stimulated glucose transport ( ,   -  ).	transcription
61209	1	336090	5	NULL	NULL	0	NULL	PMA	Chemical		stimulates					sphingolipid	Chemical	turnover of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_4_2606_s_161	15546881	On the other hand, if PMA stimulates turnover of sphingolipids resulting in the formation of sphingosine as a breakdown product which is then acylated back to ceramide, then PMA would not stimulate the acute incorporation of palmitate.	transcription
61210	2	336090	5	NULL	NULL	0	NULL	statement 1	Process		results in					sphingosine	Chemical	formation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_4_2606_s_161	15546881	On the other hand, if PMA stimulates turnover of sphingolipids resulting in the formation of sphingosine as a breakdown product which is then acylated back to ceramide, then PMA would not stimulate the acute incorporation of palmitate.	transcription
61211	3	336090	5	NULL	NULL	0	NULL	sphingosine	Chemical		acylated to					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_4_2606_s_161	15546881	On the other hand, if PMA stimulates turnover of sphingolipids resulting in the formation of sphingosine as a breakdown product which is then acylated back to ceramide, then PMA would not stimulate the acute incorporation of palmitate.	transcription
61212	4	336090	5	NULL	NULL	0	NULL	PMA	Chemical		does not stimulate					palmitate	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_4_2606_s_161	15546881	On the other hand, if PMA stimulates turnover of sphingolipids resulting in the formation of sphingosine as a breakdown product which is then acylated back to ceramide, then PMA would not stimulate the acute incorporation of palmitate.	transcription
67615	1	336090	7	NULL	NULL	0	NULL	PMA	Chemical		stimulate					sphingolipids	Chemical	turnover of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_4_2606_s_161	15546881	On the other hand, if PMA stimulates turnover of sphingolipids resulting in the formation of sphingosine as a breakdown product which is then acylated back to ceramide, then PMA would not stimulate the acute incorporation of palmitate.	transcription
67616	2	336090	7	NULL	NULL	0	NULL	statement 1	Process		result in					sphingosine	Chemical	formation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_4_2606_s_161	15546881	On the other hand, if PMA stimulates turnover of sphingolipids resulting in the formation of sphingosine as a breakdown product which is then acylated back to ceramide, then PMA would not stimulate the acute incorporation of palmitate.	transcription
67617	3	336090	7	NULL	NULL	0	NULL	sphingosine	Chemical		acylated to					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_4_2606_s_161	15546881	On the other hand, if PMA stimulates turnover of sphingolipids resulting in the formation of sphingosine as a breakdown product which is then acylated back to ceramide, then PMA would not stimulate the acute incorporation of palmitate.	transcription
67618	4	336090	7	NULL	NULL	0	NULL	sphingosine	Chemical		is a type of					breakdown product	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_4_2606_s_161	15546881	On the other hand, if PMA stimulates turnover of sphingolipids resulting in the formation of sphingosine as a breakdown product which is then acylated back to ceramide, then PMA would not stimulate the acute incorporation of palmitate.	transcription
67619	5	336090	7	NULL	NULL	NULL	NULL	PMA	Chemical		does not stimulate					palmitate	Chemical	acute incorporation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_4_2606_s_161	15546881	On the other hand, if PMA stimulates turnover of sphingolipids resulting in the formation of sphingosine as a breakdown product which is then acylated back to ceramide, then PMA would not stimulate the acute incorporation of palmitate.	transcription
61213	1	336091	5	NULL	NULL	0	NULL	Fumonisin B1	Chemical		inhibits					sphinganine/sphingosine fatty-acyl-CoA N-acyltransferase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_26680_s_143	15919667	Fumonisin B1 inhibits the sphinganine/sphingosine fatty-acyl-CoA  N-acyltransferase, blocking both ceramide synthesis  de novo and the salvage pathway ( ), whereas PPMP inhibits UDPG:CGT, the enzyme that catalyzes glucosylceramide synthesis ( ).	transcription
61214	2	336091	5	NULL	NULL	0	NULL	statement 1	Process		blocks					ceramide	Chemical	de novo synthesis of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_26680_s_143	15919667	Fumonisin B1 inhibits the sphinganine/sphingosine fatty-acyl-CoA  N-acyltransferase, blocking both ceramide synthesis  de novo and the salvage pathway ( ), whereas PPMP inhibits UDPG:CGT, the enzyme that catalyzes glucosylceramide synthesis ( ).	transcription
61215	3	336091	5	NULL	NULL	0	NULL	statement 1	Process		blocks					salvage pathway	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_26680_s_143	15919667	Fumonisin B1 inhibits the sphinganine/sphingosine fatty-acyl-CoA  N-acyltransferase, blocking both ceramide synthesis  de novo and the salvage pathway ( ), whereas PPMP inhibits UDPG:CGT, the enzyme that catalyzes glucosylceramide synthesis ( ).	transcription
61216	4	336091	5	NULL	NULL	0	NULL	PPMP	Chemical		inhibits					UDPG:CGT	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_26680_s_143	15919667	Fumonisin B1 inhibits the sphinganine/sphingosine fatty-acyl-CoA  N-acyltransferase, blocking both ceramide synthesis  de novo and the salvage pathway ( ), whereas PPMP inhibits UDPG:CGT, the enzyme that catalyzes glucosylceramide synthesis ( ).	transcription
61217	5	336091	5	NULL	NULL	0	NULL	UDPG:CGT	GP		catalyzes					glucosylceramide	Chemical	synthesis of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_26680_s_143	15919667	Fumonisin B1 inhibits the sphinganine/sphingosine fatty-acyl-CoA  N-acyltransferase, blocking both ceramide synthesis  de novo and the salvage pathway ( ), whereas PPMP inhibits UDPG:CGT, the enzyme that catalyzes glucosylceramide synthesis ( ).	transcription
67620	1	336091	7	NULL	NULL	0	NULL	Fumonisin B1	Chemical		inhibit					sphinganine fatty-acyl-CoA N-acyltransferase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_26680_s_143	15919667	Fumonisin B1 inhibits the sphinganine/sphingosine fatty-acyl-CoA  N-acyltransferase, blocking both ceramide synthesis  de novo and the salvage pathway ( ), whereas PPMP inhibits UDPG:CGT, the enzyme that catalyzes glucosylceramide synthesis ( ).	transcription
67621	2	336091	7	NULL	NULL	0	NULL	Fumonisin B1	Chemical		inhibit					sphingosine fatty-acyl-CoA N-acyltransferase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_26680_s_143	15919667	Fumonisin B1 inhibits the sphinganine/sphingosine fatty-acyl-CoA  N-acyltransferase, blocking both ceramide synthesis  de novo and the salvage pathway ( ), whereas PPMP inhibits UDPG:CGT, the enzyme that catalyzes glucosylceramide synthesis ( ).	transcription
67622	3	336091	7	NULL	NULL	0	NULL	statement 1	Process		block					ceramide synthesis	Process	de novo			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_26680_s_143	15919667	Fumonisin B1 inhibits the sphinganine/sphingosine fatty-acyl-CoA  N-acyltransferase, blocking both ceramide synthesis  de novo and the salvage pathway ( ), whereas PPMP inhibits UDPG:CGT, the enzyme that catalyzes glucosylceramide synthesis ( ).	transcription
67623	4	336091	7	NULL	NULL	0	NULL	statement 1	Process		block					ceramide synthesis	Process	salvage			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_26680_s_143	15919667	Fumonisin B1 inhibits the sphinganine/sphingosine fatty-acyl-CoA  N-acyltransferase, blocking both ceramide synthesis  de novo and the salvage pathway ( ), whereas PPMP inhibits UDPG:CGT, the enzyme that catalyzes glucosylceramide synthesis ( ).	transcription
67624	5	336091	7	NULL	NULL	0	NULL	statement 2	Process		block					ceramide synthesis	Process	de novo			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_26680_s_143	15919667	Fumonisin B1 inhibits the sphinganine/sphingosine fatty-acyl-CoA  N-acyltransferase, blocking both ceramide synthesis  de novo and the salvage pathway ( ), whereas PPMP inhibits UDPG:CGT, the enzyme that catalyzes glucosylceramide synthesis ( ).	transcription
67625	6	336091	7	NULL	NULL	0	NULL	statement 2	Process		block					ceramide synthesis	Process	salvage			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_26680_s_143	15919667	Fumonisin B1 inhibits the sphinganine/sphingosine fatty-acyl-CoA  N-acyltransferase, blocking both ceramide synthesis  de novo and the salvage pathway ( ), whereas PPMP inhibits UDPG:CGT, the enzyme that catalyzes glucosylceramide synthesis ( ).	transcription
67626	7	336091	7	NULL	NULL	0	NULL	PPMP	Chemical		inhibit					UDPG:CGT	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_26680_s_143	15919667	Fumonisin B1 inhibits the sphinganine/sphingosine fatty-acyl-CoA  N-acyltransferase, blocking both ceramide synthesis  de novo and the salvage pathway ( ), whereas PPMP inhibits UDPG:CGT, the enzyme that catalyzes glucosylceramide synthesis ( ).	transcription
67627	8	336091	7	NULL	NULL	0	NULL	UDPG:CGT	GP		catalyze					glucosylceramide synthesis	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_29_26680_s_143	15919667	Fumonisin B1 inhibits the sphinganine/sphingosine fatty-acyl-CoA  N-acyltransferase, blocking both ceramide synthesis  de novo and the salvage pathway ( ), whereas PPMP inhibits UDPG:CGT, the enzyme that catalyzes glucosylceramide synthesis ( ).	transcription
61218	1	336092	5	NULL	NULL	0	NULL	ceramide ( N-acyl sphingosine)	Chemical		is a metabolite of					sphingomyelin	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12036_s_18	14722105	For instance, one sphingomyelin metabolic product, ceramide ( N-acyl sphingosine) induces apoptosis, whereas another metabolic product, sphingosine-1-phosphate (S1P),  1 induces cell proliferation ( ,  ).	transcription
61219	2	336092	5	NULL	NULL	0	NULL	ceramide ( N-acyl sphingosine)	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12036_s_18	14722105	For instance, one sphingomyelin metabolic product, ceramide ( N-acyl sphingosine) induces apoptosis, whereas another metabolic product, sphingosine-1-phosphate (S1P),  1 induces cell proliferation ( ,  ).	transcription
61220	3	336092	5	NULL	NULL	0	NULL	S1P	Chemical		is					sphingosine-1-phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12036_s_18	14722105	For instance, one sphingomyelin metabolic product, ceramide ( N-acyl sphingosine) induces apoptosis, whereas another metabolic product, sphingosine-1-phosphate (S1P),  1 induces cell proliferation ( ,  ).	transcription
61221	4	336092	5	NULL	NULL	0	NULL	S1P	Chemical		is a metabolite of					sphingomyelin	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12036_s_18	14722105	For instance, one sphingomyelin metabolic product, ceramide ( N-acyl sphingosine) induces apoptosis, whereas another metabolic product, sphingosine-1-phosphate (S1P),  1 induces cell proliferation ( ,  ).	transcription
61222	5	336092	5	NULL	NULL	0	NULL	S1P	Chemical		induce					cell proliferation	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12036_s_18	14722105	For instance, one sphingomyelin metabolic product, ceramide ( N-acyl sphingosine) induces apoptosis, whereas another metabolic product, sphingosine-1-phosphate (S1P),  1 induces cell proliferation ( ,  ).	transcription
67628	1	336092	7	NULL	NULL	0	NULL	ceramide ( N-acyl sphingosine) 	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12036_s_18	14722105	For instance, one sphingomyelin metabolic product, ceramide ( N-acyl sphingosine) induces apoptosis, whereas another metabolic product, sphingosine-1-phosphate (S1P),  1 induces cell proliferation ( ,  ).	transcription
67629	2	336092	7	NULL	NULL	0	NULL	S1P	Chemical		induce					cell proliferation	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12036_s_18	14722105	For instance, one sphingomyelin metabolic product, ceramide ( N-acyl sphingosine) induces apoptosis, whereas another metabolic product, sphingosine-1-phosphate (S1P),  1 induces cell proliferation ( ,  ).	transcription
67630	3	336092	7	NULL	NULL	0	NULL	ceramide ( N-acyl sphingosine)	Chemical		is a metabolic product of					sphingomyelin	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12036_s_18	14722105	For instance, one sphingomyelin metabolic product, ceramide ( N-acyl sphingosine) induces apoptosis, whereas another metabolic product, sphingosine-1-phosphate (S1P),  1 induces cell proliferation ( ,  ).	transcription
67631	4	336092	7	NULL	NULL	0	NULL	S1P	Chemical		is a metabolic product of					sphingomyelin	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12036_s_18	14722105	For instance, one sphingomyelin metabolic product, ceramide ( N-acyl sphingosine) induces apoptosis, whereas another metabolic product, sphingosine-1-phosphate (S1P),  1 induces cell proliferation ( ,  ).	transcription
67632	5	336092	7	NULL	NULL	0	NULL	S1P	Chemical		is					sphingosine-1-phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_13_12036_s_18	14722105	For instance, one sphingomyelin metabolic product, ceramide ( N-acyl sphingosine) induces apoptosis, whereas another metabolic product, sphingosine-1-phosphate (S1P),  1 induces cell proliferation ( ,  ).	transcription
61223	1	336093	5	NULL	NULL	0	NULL	SK1	GP		plays a role in					S1P	Chemical	regulation of;;levels of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_34_24695_s_20	16803890	Although SK1 plays a major role, regulation of S1P levels is a function of the net responses of enzymes of the sphingolipid network that influence the levels of ceramide and sphingosine (precursors for S1P synthesis).	transcription
67633	1	336093	7	NULL	NULL	0	NULL	 S1P 	Chemical	regulation of;;levels of	is a function of					sphingolipid network	Chemical	enzymes of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_34_24695_s_20	16803890	Although SK1 plays a major role, regulation of S1P levels is a function of the net responses of enzymes of the sphingolipid network that influence the levels of ceramide and sphingosine (precursors for S1P synthesis).	transcription
67634	2	336093	7	NULL	NULL	0	NULL	ceramide	Chemical		is a precursor of					S1P synthesis	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_34_24695_s_20	16803890	Although SK1 plays a major role, regulation of S1P levels is a function of the net responses of enzymes of the sphingolipid network that influence the levels of ceramide and sphingosine (precursors for S1P synthesis).	transcription
67635	3	336093	7	NULL	NULL	0	NULL	sphingosine	Chemical		is a precursor of					S1P synthesis	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_34_24695_s_20	16803890	Although SK1 plays a major role, regulation of S1P levels is a function of the net responses of enzymes of the sphingolipid network that influence the levels of ceramide and sphingosine (precursors for S1P synthesis).	transcription
61224	1	336094	5	NULL	NULL	0	NULL	AC	GP	purified;;recombinant;;human	catalyzes					ceramide	Chemical	synthesis of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_35_32978_s_273	12815059	We therefore decided to test whether our purified, recombinant human AC  could catalyze ceramide synthesis using 14C-labeled C12  fatty acid and sphingosine as substrates.	transcription
61225	2	336094	5	NULL	NULL	0	NULL	C12 fatty acid	Chemical	14C-labeled	is a substrate for					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_35_32978_s_273	12815059	We therefore decided to test whether our purified, recombinant human AC  could catalyze ceramide synthesis using 14C-labeled C12  fatty acid and sphingosine as substrates.	transcription
61226	3	336094	5	NULL	NULL	0	NULL	sphingosine	Chemical		is a substrate for					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_35_32978_s_273	12815059	We therefore decided to test whether our purified, recombinant human AC  could catalyze ceramide synthesis using 14C-labeled C12  fatty acid and sphingosine as substrates.	transcription
61227	1	336095	5	NULL	NULL	0	NULL	C/EBP	GP		bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_11_2497_s_138	16106045	To test whether other sphingolipids in addition to ceramide might induce C/EBP DNA binding, hepatocytes were treated with 30 muM C2-dihydroceramide, sphingosine, or dihydrosphingosine (sphinganine).	transcription
61228	2	336095	5	NULL	NULL	0	NULL	ceramide	Chemical		induce					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_11_2497_s_138	16106045	To test whether other sphingolipids in addition to ceramide might induce C/EBP DNA binding, hepatocytes were treated with 30 muM C2-dihydroceramide, sphingosine, or dihydrosphingosine (sphinganine).	transcription
61229	3	336095	5	NULL	NULL	0	NULL	sphingolipids	Chemical		induce		may			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_46_11_2497_s_138	16106045	To test whether other sphingolipids in addition to ceramide might induce C/EBP DNA binding, hepatocytes were treated with 30 muM C2-dihydroceramide, sphingosine, or dihydrosphingosine (sphinganine).	transcription
61230	1	336096	5	NULL	NULL	0	NULL	S1P	Chemical		is					sphingosine 1-phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_9_1772_s_21	12777464	In contrast, its catabolic intermediate sphingosine 1-phosphate (S1P) has been implicated as a second messenger in cellular proliferation and survival ( ), and also in protection against ceramide-mediated apoptosis ( ).	transcription
61231	2	336096	5	NULL	NULL	0	NULL	S1P	Chemical		is a type of					second messenger	Chemical				NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_9_1772_s_21	12777464	In contrast, its catabolic intermediate sphingosine 1-phosphate (S1P) has been implicated as a second messenger in cellular proliferation and survival ( ), and also in protection against ceramide-mediated apoptosis ( ).	transcription
61232	3	336096	5	NULL	NULL	0	NULL	S1P	Chemical		plays a role in					cellular proliferation	Process				NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_9_1772_s_21	12777464	In contrast, its catabolic intermediate sphingosine 1-phosphate (S1P) has been implicated as a second messenger in cellular proliferation and survival ( ), and also in protection against ceramide-mediated apoptosis ( ).	transcription
61233	4	336096	5	NULL	NULL	0	NULL	S1P	Chemical		plays a role in					cell survival	Process				NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_9_1772_s_21	12777464	In contrast, its catabolic intermediate sphingosine 1-phosphate (S1P) has been implicated as a second messenger in cellular proliferation and survival ( ), and also in protection against ceramide-mediated apoptosis ( ).	transcription
61234	5	336096	5	NULL	NULL	0	NULL	apoptosis	Process		is mediated by					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_9_1772_s_21	12777464	In contrast, its catabolic intermediate sphingosine 1-phosphate (S1P) has been implicated as a second messenger in cellular proliferation and survival ( ), and also in protection against ceramide-mediated apoptosis ( ).	transcription
61235	6	336096	5	NULL	NULL	0	NULL	S1P	Chemical		protects against					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_9_1772_s_21	12777464	In contrast, its catabolic intermediate sphingosine 1-phosphate (S1P) has been implicated as a second messenger in cellular proliferation and survival ( ), and also in protection against ceramide-mediated apoptosis ( ).	transcription
67637	1	336096	7	NULL	NULL	0	NULL	S1P	Chemical		implicated as					cellular proliferation	Process	second messenger in			NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_9_1772_s_21	12777464	In contrast, its catabolic intermediate sphingosine 1-phosphate (S1P) has been implicated as a second messenger in cellular proliferation and survival ( ), and also in protection against ceramide-mediated apoptosis ( ).	transcription
67638	2	336096	7	NULL	NULL	0	NULL	S1P	Chemical		implicated as					cellular survival	Process	second messenger in			NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_9_1772_s_21	12777464	In contrast, its catabolic intermediate sphingosine 1-phosphate (S1P) has been implicated as a second messenger in cellular proliferation and survival ( ), and also in protection against ceramide-mediated apoptosis ( ).	transcription
67639	3	336096	7	NULL	NULL	0	NULL	ceramide	Chemical		mediate					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_9_1772_s_21	12777464	In contrast, its catabolic intermediate sphingosine 1-phosphate (S1P) has been implicated as a second messenger in cellular proliferation and survival ( ), and also in protection against ceramide-mediated apoptosis ( ).	transcription
67640	4	336096	7	NULL	NULL	0	NULL	S1P	Chemical		protects from					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_9_1772_s_21	12777464	In contrast, its catabolic intermediate sphingosine 1-phosphate (S1P) has been implicated as a second messenger in cellular proliferation and survival ( ), and also in protection against ceramide-mediated apoptosis ( ).	transcription
67641	5	336096	7	NULL	NULL	0	NULL	S1P	Chemical		is					sphingosine 1-phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_9_1772_s_21	12777464	In contrast, its catabolic intermediate sphingosine 1-phosphate (S1P) has been implicated as a second messenger in cellular proliferation and survival ( ), and also in protection against ceramide-mediated apoptosis ( ).	transcription
61236	1	336097	5	NULL	NULL	0	NULL	FB1	Chemical		is an inhibitor of		potent			ceramide synthase	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_305_1_232_s_188	12649374	FB1 is a potent inhibitor of sphinganine (sphingosine)  N-acetyltransferase (ceramide synthase) in vivo, and it exhibits competitive-type inhibition with respect to both substrates of this enzyme (Wang et al., 1991 ).	transcription
61237	2	336097	5	NULL	NULL	0	NULL	ceramide synthase	GP		is					sphinganine (sphingosine) N-acetyltransferase	GP				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_305_1_232_s_188	12649374	FB1 is a potent inhibitor of sphinganine (sphingosine)  N-acetyltransferase (ceramide synthase) in vivo, and it exhibits competitive-type inhibition with respect to both substrates of this enzyme (Wang et al., 1991 ).	transcription
67642	1	336097	7	NULL	NULL	NULL	NULL	FB1	Chemical		is an inhibitor of		potent			sphinganine (sphingosine) N-acetyltransferase	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_305_1_232_s_188	12649374	FB1 is a potent inhibitor of sphinganine (sphingosine)  N-acetyltransferase (ceramide synthase) in vivo, and it exhibits competitive-type inhibition with respect to both substrates of this enzyme (Wang et al., 1991 ).	transcription
67643	2	336097	7	NULL	NULL	0	NULL	sphinganine (sphingosine) N-acetyltransferase	GP		is					ceramide synthase	GP				NULL		0	NULL	NULL	NULL	gw70_jpharmacolexpther_305_1_232_s_188	12649374	FB1 is a potent inhibitor of sphinganine (sphingosine)  N-acetyltransferase (ceramide synthase) in vivo, and it exhibits competitive-type inhibition with respect to both substrates of this enzyme (Wang et al., 1991 ).	transcription
61238	1	336098	5	NULL	NULL	0	NULL	D- erythro- N-octanoyl-sphingosine	Chemical	alterations in degree and position of;;unsaturation of;;bonds in sphingoid backbone of 	affects					ceramide analogs		antiproliferative ability of 			NULL	breast cancer cells	NULL	NULL	NULL	NULL	gw70_jpharmacolexpther_309_2_523_s_3	14742741	This study demonstrates that alterations in the degree and position of unsaturation of bonds in the sphingoid backbone of D- erythro- N-octanoyl-sphingosine (Cer) affect the antiproliferative ability of ceramide analogs in breast cancer cells.	transcription
67644	1	336098	7	NULL	NULL	0	NULL	D- erythro- N-octanoyl-sphingosine (Cer)	Chemical	alterations in sphingoid backbone of	affect					ceramide analogs	Chemical	antiproliferative ability of			NULL	breast cancer cells	0	NULL	NULL	NULL	gw70_jpharmacolexpther_309_2_523_s_3	14742741	This study demonstrates that alterations in the degree and position of unsaturation of bonds in the sphingoid backbone of D- erythro- N-octanoyl-sphingosine (Cer) affect the antiproliferative ability of ceramide analogs in breast cancer cells.	transcription
67645	1	336099	7	NULL	NULL	0	NULL	Natural ceramide	Chemical		induce					c-jun	GP	expression of			NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_66	12135749	HL-60 cells were treated with the indicated concentrations of sphingosine for 1 h. C2, treated with 5  M C2-ceramide for 1 h. C: Natural ceramide-induced c-jun expression.	transcription
61239	1	336100	5	NULL	NULL	0	NULL	sphingosine	Chemical		increases					PA	Chemical	intracellular levels of			NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_12_7356_s_213	11705908	Sphingosine and sphingosine-1-phosphate increase intracellular levels of PA, thereby stimulating mitogenesis, while ceramide inhibits phospholipase D activation, thereby decreasing PA levels and enhancing the apoptotic response ( 22).	transcription
61240	2	336100	5	NULL	NULL	0	NULL	sphingosine-1-phosphate	Chemical		increases					PA	Chemical	intracellular levels of			NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_12_7356_s_213	11705908	Sphingosine and sphingosine-1-phosphate increase intracellular levels of PA, thereby stimulating mitogenesis, while ceramide inhibits phospholipase D activation, thereby decreasing PA levels and enhancing the apoptotic response ( 22).	transcription
61241	3	336100	5	NULL	NULL	0	NULL	statement 1	Process		stimulates					mitogenesis	Process				NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_12_7356_s_213	11705908	Sphingosine and sphingosine-1-phosphate increase intracellular levels of PA, thereby stimulating mitogenesis, while ceramide inhibits phospholipase D activation, thereby decreasing PA levels and enhancing the apoptotic response ( 22).	transcription
61242	4	336100	5	NULL	NULL	0	NULL	statement 2	Process		stimulates					mitogenesis	Process				NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_12_7356_s_213	11705908	Sphingosine and sphingosine-1-phosphate increase intracellular levels of PA, thereby stimulating mitogenesis, while ceramide inhibits phospholipase D activation, thereby decreasing PA levels and enhancing the apoptotic response ( 22).	transcription
61243	5	336100	5	NULL	NULL	0	NULL	ceramide	Chemical		inhibits					phospholipase D	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_12_7356_s_213	11705908	Sphingosine and sphingosine-1-phosphate increase intracellular levels of PA, thereby stimulating mitogenesis, while ceramide inhibits phospholipase D activation, thereby decreasing PA levels and enhancing the apoptotic response ( 22).	transcription
61244	6	336100	5	NULL	NULL	0	NULL	statement 5	Process		decreases					PA	Chemical	level of			NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_12_7356_s_213	11705908	Sphingosine and sphingosine-1-phosphate increase intracellular levels of PA, thereby stimulating mitogenesis, while ceramide inhibits phospholipase D activation, thereby decreasing PA levels and enhancing the apoptotic response ( 22).	transcription
61245	7	336100	5	NULL	NULL	0	NULL	statement 6	Process		enhances					apoptotic response	Process				NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_12_7356_s_213	11705908	Sphingosine and sphingosine-1-phosphate increase intracellular levels of PA, thereby stimulating mitogenesis, while ceramide inhibits phospholipase D activation, thereby decreasing PA levels and enhancing the apoptotic response ( 22).	transcription
67646	1	336100	7	NULL	NULL	0	NULL	Sphingosine	Chemical		increase					PA	Chemical	 intracellular levels of 			NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_12_7356_s_213	11705908	Sphingosine and sphingosine-1-phosphate increase intracellular levels of PA, thereby stimulating mitogenesis, while ceramide inhibits phospholipase D activation, thereby decreasing PA levels and enhancing the apoptotic response ( 22).	transcription
67647	2	336100	7	NULL	NULL	0	NULL	sphingosine-1-phosphate	Chemical		increase					PA	Chemical	intracellular levels of			NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_12_7356_s_213	11705908	Sphingosine and sphingosine-1-phosphate increase intracellular levels of PA, thereby stimulating mitogenesis, while ceramide inhibits phospholipase D activation, thereby decreasing PA levels and enhancing the apoptotic response ( 22).	transcription
67648	3	336100	7	NULL	NULL	0	NULL	statement 1	Process		stimulate					mitogenesis	Process				NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_12_7356_s_213	11705908	Sphingosine and sphingosine-1-phosphate increase intracellular levels of PA, thereby stimulating mitogenesis, while ceramide inhibits phospholipase D activation, thereby decreasing PA levels and enhancing the apoptotic response ( 22).	transcription
67649	4	336100	7	NULL	NULL	0	NULL	statement 2	Process		stimulate					mitogenesis	Process				NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_12_7356_s_213	11705908	Sphingosine and sphingosine-1-phosphate increase intracellular levels of PA, thereby stimulating mitogenesis, while ceramide inhibits phospholipase D activation, thereby decreasing PA levels and enhancing the apoptotic response ( 22).	transcription
67650	5	336100	7	NULL	NULL	0	NULL	ceramide	Chemical		inhibit					phospholipase D	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_12_7356_s_213	11705908	Sphingosine and sphingosine-1-phosphate increase intracellular levels of PA, thereby stimulating mitogenesis, while ceramide inhibits phospholipase D activation, thereby decreasing PA levels and enhancing the apoptotic response ( 22).	transcription
67651	6	336100	7	NULL	NULL	0	NULL	statement 5	Process		decrease					PA 	Chemical	levels of			NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_12_7356_s_213	11705908	Sphingosine and sphingosine-1-phosphate increase intracellular levels of PA, thereby stimulating mitogenesis, while ceramide inhibits phospholipase D activation, thereby decreasing PA levels and enhancing the apoptotic response ( 22).	transcription
67652	7	336100	7	NULL	NULL	0	NULL	statement 5	Process		enhance					apoptotic response	Process				NULL		0	NULL	NULL	NULL	gw60_infectimmun_69_12_7356_s_213	11705908	Sphingosine and sphingosine-1-phosphate increase intracellular levels of PA, thereby stimulating mitogenesis, while ceramide inhibits phospholipase D activation, thereby decreasing PA levels and enhancing the apoptotic response ( 22).	transcription
61246	1	336101	5	NULL	NULL	0	NULL	caspases	GP	active	cleave					poly(ADP-ribose) polymerase	GP				NULL	Jurkat T lymphocytes	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_135_s_210	12531546	O. Cuvillier, D.S. Rosenthal, M.E. Smulson and S. Spiegel , Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide-mediated apoptosis in Jurkat T lymphocytes.	transcription
61247	2	336101	5	NULL	NULL	0	NULL	caspases	GP	active	cleave					lamins	GP				NULL	Jurkat T lymphocytes	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_135_s_210	12531546	O. Cuvillier, D.S. Rosenthal, M.E. Smulson and S. Spiegel , Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide-mediated apoptosis in Jurkat T lymphocytes.	transcription
61248	3	336101	5	NULL	NULL	0	NULL	Sphingosine 1-phosphate	Chemical		inhibits					caspases	GP	activation of			NULL	Jurkat T lymphocytes	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_135_s_210	12531546	O. Cuvillier, D.S. Rosenthal, M.E. Smulson and S. Spiegel , Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide-mediated apoptosis in Jurkat T lymphocytes.	transcription
61249	4	336101	5	NULL	NULL	0	NULL	Fas	GP		mediates					apoptosis	Process				NULL	Jurkat T lymphocytes	0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_135_s_210	12531546	O. Cuvillier, D.S. Rosenthal, M.E. Smulson and S. Spiegel , Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide-mediated apoptosis in Jurkat T lymphocytes.	transcription
61250	5	336101	5	NULL	NULL	0	NULL	ceramide	Chemical		mediates					apoptosis	Process				NULL	Jurkat T lymphocytes	0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_135_s_210	12531546	O. Cuvillier, D.S. Rosenthal, M.E. Smulson and S. Spiegel , Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide-mediated apoptosis in Jurkat T lymphocytes.	transcription
61251	6	336101	5	NULL	NULL	0	NULL	statement 3	Process		occurs during					statement 4	Process				NULL	Jurkat T lymphocytes	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_135_s_210	12531546	O. Cuvillier, D.S. Rosenthal, M.E. Smulson and S. Spiegel , Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide-mediated apoptosis in Jurkat T lymphocytes.	transcription
61252	7	336101	5	NULL	NULL	0	NULL	statement 3	Process		occurs during					statement 5	Process				NULL	Jurkat T lymphocytes	0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_135_s_210	12531546	O. Cuvillier, D.S. Rosenthal, M.E. Smulson and S. Spiegel , Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide-mediated apoptosis in Jurkat T lymphocytes.	transcription
67653	1	336101	7	NULL	NULL	0	NULL	Sphingosine 1-phosphate	Chemical		inhibit					caspases	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_135_s_210	12531546	O. Cuvillier, D.S. Rosenthal, M.E. Smulson and S. Spiegel , Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide-mediated apoptosis in Jurkat T lymphocytes.	transcription
67654	2	336101	7	NULL	NULL	0	NULL	caspases	GP		cleave					poly(ADP-ribose) polymerase	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_135_s_210	12531546	O. Cuvillier, D.S. Rosenthal, M.E. Smulson and S. Spiegel , Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide-mediated apoptosis in Jurkat T lymphocytes.	transcription
67655	3	336101	7	NULL	NULL	0	NULL	caspases	GP		cleave					lamins	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_135_s_210	12531546	O. Cuvillier, D.S. Rosenthal, M.E. Smulson and S. Spiegel , Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide-mediated apoptosis in Jurkat T lymphocytes.	transcription
67656	4	336101	7	NULL	NULL	0	NULL	Fas	GP		mediate					apoptosis	Process				NULL	Jurkat T lymphocytes	0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_135_s_210	12531546	O. Cuvillier, D.S. Rosenthal, M.E. Smulson and S. Spiegel , Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide-mediated apoptosis in Jurkat T lymphocytes.	transcription
67657	5	336101	7	NULL	NULL	0	NULL	ceramide	Chemical		mediate					apoptosis	Process				NULL	Jurkat T lymphocytes	0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_135_s_210	12531546	O. Cuvillier, D.S. Rosenthal, M.E. Smulson and S. Spiegel , Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide-mediated apoptosis in Jurkat T lymphocytes.	transcription
67658	6	336101	7	NULL	NULL	0	NULL	statement 2	Process		occur during					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_135_s_210	12531546	O. Cuvillier, D.S. Rosenthal, M.E. Smulson and S. Spiegel , Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide-mediated apoptosis in Jurkat T lymphocytes.	transcription
67659	7	336101	7	NULL	NULL	0	NULL	statement 2	Process		occur during					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_135_s_210	12531546	O. Cuvillier, D.S. Rosenthal, M.E. Smulson and S. Spiegel , Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide-mediated apoptosis in Jurkat T lymphocytes.	transcription
67660	8	336101	7	NULL	NULL	0	NULL	statement 3	Process		occur during					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_135_s_210	12531546	O. Cuvillier, D.S. Rosenthal, M.E. Smulson and S. Spiegel , Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide-mediated apoptosis in Jurkat T lymphocytes.	transcription
67661	9	336101	7	NULL	NULL	0	NULL	statement 3	Process		occur during					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_135_s_210	12531546	O. Cuvillier, D.S. Rosenthal, M.E. Smulson and S. Spiegel , Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide-mediated apoptosis in Jurkat T lymphocytes.	transcription
61253	1	336102	5	NULL	NULL	0	NULL	neutrophils	Cell	human	treated with					TNF 	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_26	12531549	Treatment of human neutrophils with tumor necrosis factor  (TNF ) induced elevation of both intracellular ceramide and sphingosine contents during the first 60 min prior to any apoptotic morphological changes [  5.	transcription
61254	2	336102	5	NULL	NULL	0	NULL	TNF 	GP		is					tumor necrosis factor	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_26	12531549	Treatment of human neutrophils with tumor necrosis factor  (TNF ) induced elevation of both intracellular ceramide and sphingosine contents during the first 60 min prior to any apoptotic morphological changes [  5.	transcription
61255	3	336102	5	NULL	NULL	0	NULL	statement 1	Process		induce					ceramide	Chemical	elevation of;;intracellular			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_26	12531549	Treatment of human neutrophils with tumor necrosis factor  (TNF ) induced elevation of both intracellular ceramide and sphingosine contents during the first 60 min prior to any apoptotic morphological changes [  5.	transcription
61256	4	336102	5	NULL	NULL	0	NULL	statement 1	Process		induce					sphingosine	Chemical	elevation of;;intracellular			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_26	12531549	Treatment of human neutrophils with tumor necrosis factor  (TNF ) induced elevation of both intracellular ceramide and sphingosine contents during the first 60 min prior to any apoptotic morphological changes [  5.	transcription
61257	5	336102	5	NULL	NULL	0	NULL	statement 3	Process		occurs prior to					apoptotic morphological changes	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_26	12531549	Treatment of human neutrophils with tumor necrosis factor  (TNF ) induced elevation of both intracellular ceramide and sphingosine contents during the first 60 min prior to any apoptotic morphological changes [  5.	transcription
61258	6	336102	5	NULL	NULL	0	NULL	statement 4	Process		occurs prior to					apoptotic morphological changes	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_26	12531549	Treatment of human neutrophils with tumor necrosis factor  (TNF ) induced elevation of both intracellular ceramide and sphingosine contents during the first 60 min prior to any apoptotic morphological changes [  5.	transcription
67662	1	336102	7	NULL	NULL	NULL	NULL	TNF	GP		induce					ceramide	Chemical	elevation of;;intracellular			NULL	human neutrophils	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_26	12531549	Treatment of human neutrophils with tumor necrosis factor  (TNF ) induced elevation of both intracellular ceramide and sphingosine contents during the first 60 min prior to any apoptotic morphological changes [  5.	transcription
67663	2	336102	7	NULL	NULL	NULL	NULL	TNF	GP		induce					sphingosine	Chemical	elevation of;;intracellular			NULL	human neutrophils	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_153_s_26	12531549	Treatment of human neutrophils with tumor necrosis factor  (TNF ) induced elevation of both intracellular ceramide and sphingosine contents during the first 60 min prior to any apoptotic morphological changes [  5.	transcription
61259	1	336103	5	NULL	NULL	0	NULL	sphingosine	Chemical	free	is synthesized by		only			ceramide	Chemical	hydrolysis of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1485_2_63_s_377	10832090	Because free sphingosine can only be produced by ceramide hydrolysis and not by de novo biosynthesis [ 167 and   191], AC may play a critical role in the production of these important compounds and thus in the regulation of cell growth and differentiation.	transcription
61260	2	336103	5	NULL	NULL	0	NULL	AC	GP		plays a role in		critical			statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1485_2_63_s_377	10832090	Because free sphingosine can only be produced by ceramide hydrolysis and not by de novo biosynthesis [ 167 and   191], AC may play a critical role in the production of these important compounds and thus in the regulation of cell growth and differentiation.	transcription
61261	3	336103	5	NULL	NULL	0	NULL	AC	GP		plays a role in		critical			cell growth	Process	regulation of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1485_2_63_s_377	10832090	Because free sphingosine can only be produced by ceramide hydrolysis and not by de novo biosynthesis [ 167 and   191], AC may play a critical role in the production of these important compounds and thus in the regulation of cell growth and differentiation.	transcription
61262	4	336103	5	NULL	NULL	0	NULL	AC	GP		plays a role in		critical			cell differentiation	Process	regulation of			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1485_2_63_s_377	10832090	Because free sphingosine can only be produced by ceramide hydrolysis and not by de novo biosynthesis [ 167 and   191], AC may play a critical role in the production of these important compounds and thus in the regulation of cell growth and differentiation.	transcription
61263	5	336103	5	NULL	NULL	0	NULL	statement 2	Process		leads to					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1485_2_63_s_377	10832090	Because free sphingosine can only be produced by ceramide hydrolysis and not by de novo biosynthesis [ 167 and   191], AC may play a critical role in the production of these important compounds and thus in the regulation of cell growth and differentiation.	transcription
61264	6	336103	5	NULL	NULL	0	NULL	statement 2	Process		leads to					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1485_2_63_s_377	10832090	Because free sphingosine can only be produced by ceramide hydrolysis and not by de novo biosynthesis [ 167 and   191], AC may play a critical role in the production of these important compounds and thus in the regulation of cell growth and differentiation.	transcription
67664	1	336103	7	NULL	NULL	NULL	NULL	sphingosine	GP	free	produced by					ceramide	Chemical	hydrolysis of			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1485_2_63_s_377	10832090	Because free sphingosine can only be produced by ceramide hydrolysis and not by de novo biosynthesis [ 167 and   191], AC may play a critical role in the production of these important compounds and thus in the regulation of cell growth and differentiation.	transcription
67665	2	336103	7	NULL	NULL	0	NULL	sphingosine	Chemical	free	is not produced by					de novo biosynthesis	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1485_2_63_s_377	10832090	Because free sphingosine can only be produced by ceramide hydrolysis and not by de novo biosynthesis [ 167 and   191], AC may play a critical role in the production of these important compounds and thus in the regulation of cell growth and differentiation.	transcription
67666	3	336103	7	NULL	NULL	0	NULL	AC	GP		play a critical role in					sphingosine	Chemical	production of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1485_2_63_s_377	10832090	Because free sphingosine can only be produced by ceramide hydrolysis and not by de novo biosynthesis [ 167 and   191], AC may play a critical role in the production of these important compounds and thus in the regulation of cell growth and differentiation.	transcription
67667	4	336103	7	NULL	NULL	0	NULL	statement 3	Process		play a role in					cell growth	Process	regulation of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1485_2_63_s_377	10832090	Because free sphingosine can only be produced by ceramide hydrolysis and not by de novo biosynthesis [ 167 and   191], AC may play a critical role in the production of these important compounds and thus in the regulation of cell growth and differentiation.	transcription
67668	5	336103	7	NULL	NULL	0	NULL	statement 3	Process		play a role in					cell differentiation	Process	regulation of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1485_2_63_s_377	10832090	Because free sphingosine can only be produced by ceramide hydrolysis and not by de novo biosynthesis [ 167 and   191], AC may play a critical role in the production of these important compounds and thus in the regulation of cell growth and differentiation.	transcription
61265	1	336104	5	NULL	NULL	0	NULL	cell death	Process		is induced by					TNF	GP				NULL	promyeloid U937 cells	0	NULL	NULL	NULL	gw60_biochimbiophysacta_1485_2_63_s_496	10832090	Obeid et al. were the first to show that an exogenously added cell-permeable short-chain ceramide analog,  N-acetyl-sphingosine, mimicked TNF -induced cell death in promyeloid U937 cells [  270].	transcription
61266	2	336104	5	NULL	NULL	0	NULL	N-acetyl-sphingosine	Chemical	exogenously added;;cell-permeable	mimics					statement 1					NULL	promyeloid U937 cells	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1485_2_63_s_496	10832090	Obeid et al. were the first to show that an exogenously added cell-permeable short-chain ceramide analog,  N-acetyl-sphingosine, mimicked TNF -induced cell death in promyeloid U937 cells [  270].	transcription
61267	3	336104	5	NULL	NULL	0	NULL	N-acetyl-sphingosine	Chemical		is an analog of					short-chain ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1485_2_63_s_496	10832090	Obeid et al. were the first to show that an exogenously added cell-permeable short-chain ceramide analog,  N-acetyl-sphingosine, mimicked TNF -induced cell death in promyeloid U937 cells [  270].	transcription
67669	1	336104	7	NULL	NULL	0	NULL	 TNF	GP		induce					cell death	Process				NULL	promyeloid U937 cells	0	NULL	NULL	NULL	gw60_biochimbiophysacta_1485_2_63_s_496	10832090	Obeid et al. were the first to show that an exogenously added cell-permeable short-chain ceramide analog,  N-acetyl-sphingosine, mimicked TNF -induced cell death in promyeloid U937 cells [  270].	transcription
67670	2	336104	7	NULL	NULL	0	NULL	N-acetyl-sphingosine	Chemical		mimick					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1485_2_63_s_496	10832090	Obeid et al. were the first to show that an exogenously added cell-permeable short-chain ceramide analog,  N-acetyl-sphingosine, mimicked TNF -induced cell death in promyeloid U937 cells [  270].	transcription
67671	3	336104	7	NULL	NULL	0	NULL	N-acetyl-sphingosine	Chemical		is a type of					cell-permeable short-chain ceramide analog	Chemical				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1485_2_63_s_496	10832090	Obeid et al. were the first to show that an exogenously added cell-permeable short-chain ceramide analog,  N-acetyl-sphingosine, mimicked TNF -induced cell death in promyeloid U937 cells [  270].	transcription
61268	1	336105	5	NULL	NULL	0	NULL	S1P	Chemical		ligand for		high affinity			S1P2/EDG-5	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_72_s_90	12069812	S1P is a high affinity ligand (Kd 16-27 nM) for S1P2/EDG-5 [ 7,  15,  19 and   43] and the binding of S1P to S1P2/EDG-5 can be competed by dihydro-S1P but not by sphingosine, sphingomyelin, homophosphonate S1P, ceramide, ceramide-1-phosphate or LPA [ 19 and  43].	transcription
61269	2	336105	5	NULL	NULL	0	NULL	S1P	Chemical		bind					S1P2/EDG-5	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_72_s_90	12069812	S1P is a high affinity ligand (Kd 16-27 nM) for S1P2/EDG-5 [ 7,  15,  19 and   43] and the binding of S1P to S1P2/EDG-5 can be competed by dihydro-S1P but not by sphingosine, sphingomyelin, homophosphonate S1P, ceramide, ceramide-1-phosphate or LPA [ 19 and  43].	transcription
61270	3	336105	5	NULL	NULL	0	NULL	dihydro-S1P	Chemical		bind					S1P2/EDG-5	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_72_s_90	12069812	S1P is a high affinity ligand (Kd 16-27 nM) for S1P2/EDG-5 [ 7,  15,  19 and   43] and the binding of S1P to S1P2/EDG-5 can be competed by dihydro-S1P but not by sphingosine, sphingomyelin, homophosphonate S1P, ceramide, ceramide-1-phosphate or LPA [ 19 and  43].	transcription
61271	4	336105	5	NULL	NULL	0	NULL	statement 3	Process		competes with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_72_s_90	12069812	S1P is a high affinity ligand (Kd 16-27 nM) for S1P2/EDG-5 [ 7,  15,  19 and   43] and the binding of S1P to S1P2/EDG-5 can be competed by dihydro-S1P but not by sphingosine, sphingomyelin, homophosphonate S1P, ceramide, ceramide-1-phosphate or LPA [ 19 and  43].	transcription
61272	5	336105	5	NULL	NULL	0	NULL	sphingosine	Chemical		does not compete with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_72_s_90	12069812	S1P is a high affinity ligand (Kd 16-27 nM) for S1P2/EDG-5 [ 7,  15,  19 and   43] and the binding of S1P to S1P2/EDG-5 can be competed by dihydro-S1P but not by sphingosine, sphingomyelin, homophosphonate S1P, ceramide, ceramide-1-phosphate or LPA [ 19 and  43].	transcription
61273	6	336105	5	NULL	NULL	0	NULL	sphingomyelin	Chemical		does not compete with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_72_s_90	12069812	S1P is a high affinity ligand (Kd 16-27 nM) for S1P2/EDG-5 [ 7,  15,  19 and   43] and the binding of S1P to S1P2/EDG-5 can be competed by dihydro-S1P but not by sphingosine, sphingomyelin, homophosphonate S1P, ceramide, ceramide-1-phosphate or LPA [ 19 and  43].	transcription
61274	7	336105	5	NULL	NULL	0	NULL	homophosphonate S1P	Chemical		does not compete with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_72_s_90	12069812	S1P is a high affinity ligand (Kd 16-27 nM) for S1P2/EDG-5 [ 7,  15,  19 and   43] and the binding of S1P to S1P2/EDG-5 can be competed by dihydro-S1P but not by sphingosine, sphingomyelin, homophosphonate S1P, ceramide, ceramide-1-phosphate or LPA [ 19 and  43].	transcription
61275	8	336105	5	NULL	NULL	0	NULL	ceramide	Process		does not compete with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_72_s_90	12069812	S1P is a high affinity ligand (Kd 16-27 nM) for S1P2/EDG-5 [ 7,  15,  19 and   43] and the binding of S1P to S1P2/EDG-5 can be competed by dihydro-S1P but not by sphingosine, sphingomyelin, homophosphonate S1P, ceramide, ceramide-1-phosphate or LPA [ 19 and  43].	transcription
61276	9	336105	5	NULL	NULL	0	NULL	ceramide-1-phosphate	Chemical		does not compete with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_72_s_90	12069812	S1P is a high affinity ligand (Kd 16-27 nM) for S1P2/EDG-5 [ 7,  15,  19 and   43] and the binding of S1P to S1P2/EDG-5 can be competed by dihydro-S1P but not by sphingosine, sphingomyelin, homophosphonate S1P, ceramide, ceramide-1-phosphate or LPA [ 19 and  43].	transcription
61277	10	336105	5	NULL	NULL	0	NULL	LPA	Chemical		does not compete with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_72_s_90	12069812	S1P is a high affinity ligand (Kd 16-27 nM) for S1P2/EDG-5 [ 7,  15,  19 and   43] and the binding of S1P to S1P2/EDG-5 can be competed by dihydro-S1P but not by sphingosine, sphingomyelin, homophosphonate S1P, ceramide, ceramide-1-phosphate or LPA [ 19 and  43].	transcription
67672	1	336105	7	NULL	NULL	NULL	NULL	S1P	Chemical		ligand for		high affinity			S1P2/EDG-5	GP				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_72_s_90	12069812	S1P is a high affinity ligand (Kd 16-27 nM) for S1P2/EDG-5 [ 7,  15,  19 and   43] and the binding of S1P to S1P2/EDG-5 can be competed by dihydro-S1P but not by sphingosine, sphingomyelin, homophosphonate S1P, ceramide, ceramide-1-phosphate or LPA [ 19 and  43].	transcription
67673	2	336105	7	NULL	NULL	0	NULL	S1P	Chemical		bind					S1P2/EDG-5	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_72_s_90	12069812	S1P is a high affinity ligand (Kd 16-27 nM) for S1P2/EDG-5 [ 7,  15,  19 and   43] and the binding of S1P to S1P2/EDG-5 can be competed by dihydro-S1P but not by sphingosine, sphingomyelin, homophosphonate S1P, ceramide, ceramide-1-phosphate or LPA [ 19 and  43].	transcription
67674	3	336105	7	NULL	NULL	0	NULL	dihydro-S1P	Chemical		bind					S1P2/EDG-5	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_72_s_90	12069812	S1P is a high affinity ligand (Kd 16-27 nM) for S1P2/EDG-5 [ 7,  15,  19 and   43] and the binding of S1P to S1P2/EDG-5 can be competed by dihydro-S1P but not by sphingosine, sphingomyelin, homophosphonate S1P, ceramide, ceramide-1-phosphate or LPA [ 19 and  43].	transcription
67675	4	336105	7	NULL	NULL	0	NULL	statement 3	Process		compete with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_72_s_90	12069812	S1P is a high affinity ligand (Kd 16-27 nM) for S1P2/EDG-5 [ 7,  15,  19 and   43] and the binding of S1P to S1P2/EDG-5 can be competed by dihydro-S1P but not by sphingosine, sphingomyelin, homophosphonate S1P, ceramide, ceramide-1-phosphate or LPA [ 19 and  43].	transcription
67676	5	336105	7	NULL	NULL	0	NULL	sphingosine	Chemical		does not compete with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_72_s_90	12069812	S1P is a high affinity ligand (Kd 16-27 nM) for S1P2/EDG-5 [ 7,  15,  19 and   43] and the binding of S1P to S1P2/EDG-5 can be competed by dihydro-S1P but not by sphingosine, sphingomyelin, homophosphonate S1P, ceramide, ceramide-1-phosphate or LPA [ 19 and  43].	transcription
67677	6	336105	7	NULL	NULL	0	NULL	sphingomyelin	Chemical		does not compete with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_72_s_90	12069812	S1P is a high affinity ligand (Kd 16-27 nM) for S1P2/EDG-5 [ 7,  15,  19 and   43] and the binding of S1P to S1P2/EDG-5 can be competed by dihydro-S1P but not by sphingosine, sphingomyelin, homophosphonate S1P, ceramide, ceramide-1-phosphate or LPA [ 19 and  43].	transcription
67678	7	336105	7	NULL	NULL	0	NULL	homophosphonate S1P	Chemical		does not compete with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_72_s_90	12069812	S1P is a high affinity ligand (Kd 16-27 nM) for S1P2/EDG-5 [ 7,  15,  19 and   43] and the binding of S1P to S1P2/EDG-5 can be competed by dihydro-S1P but not by sphingosine, sphingomyelin, homophosphonate S1P, ceramide, ceramide-1-phosphate or LPA [ 19 and  43].	transcription
67679	8	336105	7	NULL	NULL	0	NULL	ceramide	Chemical		does not compete with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_72_s_90	12069812	S1P is a high affinity ligand (Kd 16-27 nM) for S1P2/EDG-5 [ 7,  15,  19 and   43] and the binding of S1P to S1P2/EDG-5 can be competed by dihydro-S1P but not by sphingosine, sphingomyelin, homophosphonate S1P, ceramide, ceramide-1-phosphate or LPA [ 19 and  43].	transcription
67680	9	336105	7	NULL	NULL	0	NULL	ceramide-1-phosphate	Chemical		does not compete with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_72_s_90	12069812	S1P is a high affinity ligand (Kd 16-27 nM) for S1P2/EDG-5 [ 7,  15,  19 and   43] and the binding of S1P to S1P2/EDG-5 can be competed by dihydro-S1P but not by sphingosine, sphingomyelin, homophosphonate S1P, ceramide, ceramide-1-phosphate or LPA [ 19 and  43].	transcription
67681	10	336105	7	NULL	NULL	0	NULL	LPA	Chemical		does not compete with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_72_s_90	12069812	S1P is a high affinity ligand (Kd 16-27 nM) for S1P2/EDG-5 [ 7,  15,  19 and   43] and the binding of S1P to S1P2/EDG-5 can be competed by dihydro-S1P but not by sphingosine, sphingomyelin, homophosphonate S1P, ceramide, ceramide-1-phosphate or LPA [ 19 and  43].	transcription
66572	1	336106	5	NULL	NULL	NULL	NULL	SPP	Chemical		leads to					angiogenic responses	Process				NULL	cells treated with sphingolipids	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_228_s_56	12069833	Treatment of cells with related sphingolipids, including sphingosine, sphingomyelin, ceramide and ceramide-1-phosphate, or instillation of SPP into the cytoplasm by microinjection had no effect, demonstrating that the angiogenic responses to SPP resulted from ligation of specific cell surface receptors.	transcription
66573	2	336106	5	NULL	NULL	NULL	NULL	cell surface receptors	GP	ligation of;;specific	results in					statement 1	Process				NULL	cells treated with sphingolipids	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_228_s_56	12069833	Treatment of cells with related sphingolipids, including sphingosine, sphingomyelin, ceramide and ceramide-1-phosphate, or instillation of SPP into the cytoplasm by microinjection had no effect, demonstrating that the angiogenic responses to SPP resulted from ligation of specific cell surface receptors.	transcription
66574	3	336106	5	NULL	NULL	0	NULL	sphingosine	Chemical		is a type of					sphingolipid	Chemical				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_228_s_56	12069833	Treatment of cells with related sphingolipids, including sphingosine, sphingomyelin, ceramide and ceramide-1-phosphate, or instillation of SPP into the cytoplasm by microinjection had no effect, demonstrating that the angiogenic responses to SPP resulted from ligation of specific cell surface receptors.	transcription
66575	4	336106	5	NULL	NULL	0	NULL	sphingomyelin	Chemical		is a type of					sphingolipid	Chemical				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_228_s_56	12069833	Treatment of cells with related sphingolipids, including sphingosine, sphingomyelin, ceramide and ceramide-1-phosphate, or instillation of SPP into the cytoplasm by microinjection had no effect, demonstrating that the angiogenic responses to SPP resulted from ligation of specific cell surface receptors.	transcription
66576	5	336106	5	NULL	NULL	0	NULL	ceramide	Chemical		is a type of					sphingolipid	Chemical				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_228_s_56	12069833	Treatment of cells with related sphingolipids, including sphingosine, sphingomyelin, ceramide and ceramide-1-phosphate, or instillation of SPP into the cytoplasm by microinjection had no effect, demonstrating that the angiogenic responses to SPP resulted from ligation of specific cell surface receptors.	transcription
66577	6	336106	5	NULL	NULL	0	NULL	ceramide-1-phosphate	Chemical		is a type of					sphingolipid	Chemical				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_228_s_56	12069833	Treatment of cells with related sphingolipids, including sphingosine, sphingomyelin, ceramide and ceramide-1-phosphate, or instillation of SPP into the cytoplasm by microinjection had no effect, demonstrating that the angiogenic responses to SPP resulted from ligation of specific cell surface receptors.	transcription
67682	1	336106	7	NULL	NULL	0	NULL	SPP	Chemical	angiogenic responses to	result from					cell surface receptors	GP	ligation of specific			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1582_1_228_s_56	12069833	Treatment of cells with related sphingolipids, including sphingosine, sphingomyelin, ceramide and ceramide-1-phosphate, or instillation of SPP into the cytoplasm by microinjection had no effect, demonstrating that the angiogenic responses to SPP resulted from ligation of specific cell surface receptors.	transcription
66578	1	336107	5	NULL	NULL	0	NULL	MAPP	Chemical		is an inhibitor of					ceramidase	GP				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_2_417_s_145	11815377	This was further supported by experiments with the ceramidase inhibitor, MAPP (Bielawska  et al., 1996  ) which prevents formation of sphingosine and sphingosine-1-phosphate from ceramide and causes accumulation of the latter (Bielawska  et al., 1996  ; Hannun & Luberto, 2000  ).	transcription
66579	2	336107	5	NULL	NULL	0	NULL	sphingosine	Chemical		is formed from					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_2_417_s_145	11815377	This was further supported by experiments with the ceramidase inhibitor, MAPP (Bielawska  et al., 1996  ) which prevents formation of sphingosine and sphingosine-1-phosphate from ceramide and causes accumulation of the latter (Bielawska  et al., 1996  ; Hannun & Luberto, 2000  ).	transcription
66580	3	336107	5	NULL	NULL	0	NULL	sphingosine 1-phosphate	Chemical		is formed from					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_2_417_s_145	11815377	This was further supported by experiments with the ceramidase inhibitor, MAPP (Bielawska  et al., 1996  ) which prevents formation of sphingosine and sphingosine-1-phosphate from ceramide and causes accumulation of the latter (Bielawska  et al., 1996  ; Hannun & Luberto, 2000  ).	transcription
66581	4	336107	5	NULL	NULL	0	NULL	statement 2	Process		occurs along with					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_2_417_s_145	11815377	This was further supported by experiments with the ceramidase inhibitor, MAPP (Bielawska  et al., 1996  ) which prevents formation of sphingosine and sphingosine-1-phosphate from ceramide and causes accumulation of the latter (Bielawska  et al., 1996  ; Hannun & Luberto, 2000  ).	transcription
66583	5	336107	5	NULL	NULL	0	NULL	MAPP	Chemical		prevents					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_2_417_s_145	11815377	This was further supported by experiments with the ceramidase inhibitor, MAPP (Bielawska  et al., 1996  ) which prevents formation of sphingosine and sphingosine-1-phosphate from ceramide and causes accumulation of the latter (Bielawska  et al., 1996  ; Hannun & Luberto, 2000  ).	transcription
66584	6	336107	5	NULL	NULL	0	NULL	statement 5	Process		accumulates					sphingosine 1-phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_2_417_s_145	11815377	This was further supported by experiments with the ceramidase inhibitor, MAPP (Bielawska  et al., 1996  ) which prevents formation of sphingosine and sphingosine-1-phosphate from ceramide and causes accumulation of the latter (Bielawska  et al., 1996  ; Hannun & Luberto, 2000  ).	transcription
67684	1	336107	7	NULL	NULL	0	NULL	MAPP	Chemical		is a type of					ceramidase inhibitor	Chemical				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_2_417_s_145	11815377	This was further supported by experiments with the ceramidase inhibitor, MAPP (Bielawska  et al., 1996  ) which prevents formation of sphingosine and sphingosine-1-phosphate from ceramide and causes accumulation of the latter (Bielawska  et al., 1996  ; Hannun & Luberto, 2000  ).	transcription
67685	2	336107	7	NULL	NULL	0	NULL	sphingosine	Chemical		formed from					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_2_417_s_145	11815377	This was further supported by experiments with the ceramidase inhibitor, MAPP (Bielawska  et al., 1996  ) which prevents formation of sphingosine and sphingosine-1-phosphate from ceramide and causes accumulation of the latter (Bielawska  et al., 1996  ; Hannun & Luberto, 2000  ).	transcription
67686	3	336107	7	NULL	NULL	0	NULL	sphingosine-1-phosphate	Chemical		formed from					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_2_417_s_145	11815377	This was further supported by experiments with the ceramidase inhibitor, MAPP (Bielawska  et al., 1996  ) which prevents formation of sphingosine and sphingosine-1-phosphate from ceramide and causes accumulation of the latter (Bielawska  et al., 1996  ; Hannun & Luberto, 2000  ).	transcription
67687	4	336107	7	NULL	NULL	0	NULL	MAPP	Chemical		prevents					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_2_417_s_145	11815377	This was further supported by experiments with the ceramidase inhibitor, MAPP (Bielawska  et al., 1996  ) which prevents formation of sphingosine and sphingosine-1-phosphate from ceramide and causes accumulation of the latter (Bielawska  et al., 1996  ; Hannun & Luberto, 2000  ).	transcription
67688	5	336107	7	NULL	NULL	0	NULL	MAPP	Chemical		prevents					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_2_417_s_145	11815377	This was further supported by experiments with the ceramidase inhibitor, MAPP (Bielawska  et al., 1996  ) which prevents formation of sphingosine and sphingosine-1-phosphate from ceramide and causes accumulation of the latter (Bielawska  et al., 1996  ; Hannun & Luberto, 2000  ).	transcription
67709	6	336107	7	NULL	NULL	0	NULL	MAPP	Chemical		cause					ceramide	Chemical	accumulation of			NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_135_2_417_s_145	11815377	This was further supported by experiments with the ceramidase inhibitor, MAPP (Bielawska  et al., 1996  ) which prevents formation of sphingosine and sphingosine-1-phosphate from ceramide and causes accumulation of the latter (Bielawska  et al., 1996  ; Hannun & Luberto, 2000  ).	transcription
66596	1	336108	5	NULL	NULL	NULL	NULL	apoptosis	Process		is induced by					serum deprivation	Process				NULL	Jurkat T cells	NULL	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_13	10545499	In Jurkat T cells, overexpression of sphingosine kinase also suppressed serum deprivation- and ceramide-induced apoptosis and, to a lesser extent, Fas-induced apoptosis, which correlated with inhibition of DEVDase activity, as well as inhibition of the executionary caspase-3.	transcription
66597	2	336108	5	NULL	NULL	NULL	NULL	apoptosis	Process		is induced by					ceramide	Chemical				NULL	Jurkat T cells	NULL	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_13	10545499	In Jurkat T cells, overexpression of sphingosine kinase also suppressed serum deprivation- and ceramide-induced apoptosis and, to a lesser extent, Fas-induced apoptosis, which correlated with inhibition of DEVDase activity, as well as inhibition of the executionary caspase-3.	transcription
66598	3	336108	5	NULL	NULL	NULL	NULL	apoptosis	Process		is induced by					Fas	GP				NULL	Jurkat T cells	NULL	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_13	10545499	In Jurkat T cells, overexpression of sphingosine kinase also suppressed serum deprivation- and ceramide-induced apoptosis and, to a lesser extent, Fas-induced apoptosis, which correlated with inhibition of DEVDase activity, as well as inhibition of the executionary caspase-3.	transcription
66599	4	336108	5	NULL	NULL	0	NULL	sphingosine kinase	GP	overexpression of	suppress					statement 1	Process				NULL	Jurkat T cells	0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_13	10545499	In Jurkat T cells, overexpression of sphingosine kinase also suppressed serum deprivation- and ceramide-induced apoptosis and, to a lesser extent, Fas-induced apoptosis, which correlated with inhibition of DEVDase activity, as well as inhibition of the executionary caspase-3.	transcription
66600	5	336108	5	NULL	NULL	0	NULL	sphingosine kinase	GP	overexpression of	suppress					statement 2	Process				NULL	Jurkat T cells	0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_13	10545499	In Jurkat T cells, overexpression of sphingosine kinase also suppressed serum deprivation- and ceramide-induced apoptosis and, to a lesser extent, Fas-induced apoptosis, which correlated with inhibition of DEVDase activity, as well as inhibition of the executionary caspase-3.	transcription
66601	6	336108	5	NULL	NULL	NULL	NULL	sphingosine kinase	GP	overexpression of	suppress					statement 3	Process				NULL	Jurkat T cells	NULL	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_13	10545499	In Jurkat T cells, overexpression of sphingosine kinase also suppressed serum deprivation- and ceramide-induced apoptosis and, to a lesser extent, Fas-induced apoptosis, which correlated with inhibition of DEVDase activity, as well as inhibition of the executionary caspase-3.	transcription
66602	7	336108	5	NULL	NULL	0	NULL	statement 6	Process		lesser extent than					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_13	10545499	In Jurkat T cells, overexpression of sphingosine kinase also suppressed serum deprivation- and ceramide-induced apoptosis and, to a lesser extent, Fas-induced apoptosis, which correlated with inhibition of DEVDase activity, as well as inhibition of the executionary caspase-3.	transcription
66603	8	336108	5	NULL	NULL	0	NULL	statement 6	Process		lesser extent than					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_13	10545499	In Jurkat T cells, overexpression of sphingosine kinase also suppressed serum deprivation- and ceramide-induced apoptosis and, to a lesser extent, Fas-induced apoptosis, which correlated with inhibition of DEVDase activity, as well as inhibition of the executionary caspase-3.	transcription
66604	9	336108	5	NULL	NULL	NULL	NULL	statement 6	Process		corelates with					DEVDase	GP	inhibition of;;activity of			NULL	Jurkat T cells	NULL	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_13	10545499	In Jurkat T cells, overexpression of sphingosine kinase also suppressed serum deprivation- and ceramide-induced apoptosis and, to a lesser extent, Fas-induced apoptosis, which correlated with inhibition of DEVDase activity, as well as inhibition of the executionary caspase-3.	transcription
66605	10	336108	5	NULL	NULL	NULL	NULL	statement 6	Process		corelates with					executionary caspase-3	GP	inhibition of			NULL	Jurkat T cells	NULL	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_13	10545499	In Jurkat T cells, overexpression of sphingosine kinase also suppressed serum deprivation- and ceramide-induced apoptosis and, to a lesser extent, Fas-induced apoptosis, which correlated with inhibition of DEVDase activity, as well as inhibition of the executionary caspase-3.	transcription
67689	1	336108	7	NULL	NULL	NULL	NULL	sphingosine kinase	GP	overexpression of	suppress					serum deprivation	Process				NULL	Jurkat T cells	NULL	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_13	10545499	In Jurkat T cells, overexpression of sphingosine kinase also suppressed serum deprivation- and ceramide-induced apoptosis and, to a lesser extent, Fas-induced apoptosis, which correlated with inhibition of DEVDase activity, as well as inhibition of the executionary caspase-3.	transcription
67690	2	336108	7	NULL	NULL	0	NULL	ceramide	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_13	10545499	In Jurkat T cells, overexpression of sphingosine kinase also suppressed serum deprivation- and ceramide-induced apoptosis and, to a lesser extent, Fas-induced apoptosis, which correlated with inhibition of DEVDase activity, as well as inhibition of the executionary caspase-3.	transcription
67691	3	336108	7	NULL	NULL	NULL	NULL	sphingosine kinase	GP	overexpression of	suppress					statement 2	Process				NULL	Jurkat T cells	NULL	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_13	10545499	In Jurkat T cells, overexpression of sphingosine kinase also suppressed serum deprivation- and ceramide-induced apoptosis and, to a lesser extent, Fas-induced apoptosis, which correlated with inhibition of DEVDase activity, as well as inhibition of the executionary caspase-3.	transcription
67692	4	336108	7	NULL	NULL	0	NULL	Fas	GP		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_13	10545499	In Jurkat T cells, overexpression of sphingosine kinase also suppressed serum deprivation- and ceramide-induced apoptosis and, to a lesser extent, Fas-induced apoptosis, which correlated with inhibition of DEVDase activity, as well as inhibition of the executionary caspase-3.	transcription
67693	5	336108	7	NULL	NULL	NULL	NULL	sphingosine kinase	GP	overexpression of	suppress					statement 4	Process				NULL	Jurkat T cells	NULL	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_13	10545499	In Jurkat T cells, overexpression of sphingosine kinase also suppressed serum deprivation- and ceramide-induced apoptosis and, to a lesser extent, Fas-induced apoptosis, which correlated with inhibition of DEVDase activity, as well as inhibition of the executionary caspase-3.	transcription
67694	6	336108	7	NULL	NULL	0	NULL	statement 4	Process	suppression of	occur to a lesser extent than					statement 2	Process	suppression of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_13	10545499	In Jurkat T cells, overexpression of sphingosine kinase also suppressed serum deprivation- and ceramide-induced apoptosis and, to a lesser extent, Fas-induced apoptosis, which correlated with inhibition of DEVDase activity, as well as inhibition of the executionary caspase-3.	transcription
67695	7	336108	7	NULL	NULL	0	NULL	statement 6	Process		correlates with					DEVDase activity	Process	inhibition of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_13	10545499	In Jurkat T cells, overexpression of sphingosine kinase also suppressed serum deprivation- and ceramide-induced apoptosis and, to a lesser extent, Fas-induced apoptosis, which correlated with inhibition of DEVDase activity, as well as inhibition of the executionary caspase-3.	transcription
67696	8	336108	7	NULL	NULL	NULL	NULL	statement 6	Process		correlates with					caspase-3	GP	inhibition of;;executionary			NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_13	10545499	In Jurkat T cells, overexpression of sphingosine kinase also suppressed serum deprivation- and ceramide-induced apoptosis and, to a lesser extent, Fas-induced apoptosis, which correlated with inhibition of DEVDase activity, as well as inhibition of the executionary caspase-3.	transcription
66606	1	336109	5	NULL	NULL	0	NULL	sphingosine kinase	GP	overexpression of	increases					SPP	Chemical	levels of;;intracellular			NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_33	10545499	In this study, we demonstrate that overexpression of sphingosine kinase markedly increased intracellular mass levels of SPP, enhanced proliferation by promoting the G1 to S phase transition, and suppressed serum deprivation- and ceramide-induced apoptosis.	transcription
66607	2	336109	5	NULL	NULL	0	NULL	sphingosine kinase	GP	overexpression of	enhances					cellular proliferation	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_33	10545499	In this study, we demonstrate that overexpression of sphingosine kinase markedly increased intracellular mass levels of SPP, enhanced proliferation by promoting the G1 to S phase transition, and suppressed serum deprivation- and ceramide-induced apoptosis.	transcription
66608	3	336109	5	NULL	NULL	NULL	NULL	cell	Cell		undergoes transition from					G1 phase	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_33	10545499	In this study, we demonstrate that overexpression of sphingosine kinase markedly increased intracellular mass levels of SPP, enhanced proliferation by promoting the G1 to S phase transition, and suppressed serum deprivation- and ceramide-induced apoptosis.	transcription
66609	4	336109	5	NULL	NULL	NULL	NULL	cell	Cell		undergoes transition to					S phase	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_33	10545499	In this study, we demonstrate that overexpression of sphingosine kinase markedly increased intracellular mass levels of SPP, enhanced proliferation by promoting the G1 to S phase transition, and suppressed serum deprivation- and ceramide-induced apoptosis.	transcription
66610	5	336109	5	NULL	NULL	0	NULL	statement 3	Process		occurs along with					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_33	10545499	In this study, we demonstrate that overexpression of sphingosine kinase markedly increased intracellular mass levels of SPP, enhanced proliferation by promoting the G1 to S phase transition, and suppressed serum deprivation- and ceramide-induced apoptosis.	transcription
66611	6	336109	5	NULL	NULL	NULL	NULL	sphingosine kinase	GP	overexpression of	promotes					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_33	10545499	In this study, we demonstrate that overexpression of sphingosine kinase markedly increased intracellular mass levels of SPP, enhanced proliferation by promoting the G1 to S phase transition, and suppressed serum deprivation- and ceramide-induced apoptosis.	transcription
66612	7	336109	5	NULL	NULL	0	NULL	apoptosis	Process		is induced by					serum deprivation	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_33	10545499	In this study, we demonstrate that overexpression of sphingosine kinase markedly increased intracellular mass levels of SPP, enhanced proliferation by promoting the G1 to S phase transition, and suppressed serum deprivation- and ceramide-induced apoptosis.	transcription
66613	8	336109	5	NULL	NULL	0	NULL	apoptosis	Process		is induced by					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_33	10545499	In this study, we demonstrate that overexpression of sphingosine kinase markedly increased intracellular mass levels of SPP, enhanced proliferation by promoting the G1 to S phase transition, and suppressed serum deprivation- and ceramide-induced apoptosis.	transcription
66614	9	336109	5	NULL	NULL	0	NULL	sphingosine kinase	GP	overexpression of	suppress					statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_33	10545499	In this study, we demonstrate that overexpression of sphingosine kinase markedly increased intracellular mass levels of SPP, enhanced proliferation by promoting the G1 to S phase transition, and suppressed serum deprivation- and ceramide-induced apoptosis.	transcription
66615	10	336109	5	NULL	NULL	0	NULL	sphingosine kinase	GP	overexpression of	suppress					statement 8	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_33	10545499	In this study, we demonstrate that overexpression of sphingosine kinase markedly increased intracellular mass levels of SPP, enhanced proliferation by promoting the G1 to S phase transition, and suppressed serum deprivation- and ceramide-induced apoptosis.	transcription
66616	11	336109	5	NULL	NULL	0	NULL	statement 6	Process		leads to					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_33	10545499	In this study, we demonstrate that overexpression of sphingosine kinase markedly increased intracellular mass levels of SPP, enhanced proliferation by promoting the G1 to S phase transition, and suppressed serum deprivation- and ceramide-induced apoptosis.	transcription
67697	1	336109	7	NULL	NULL	0	NULL	sphingosine kinase	GP	overexpression of	increase		markedly			SPP	Chemical	intracellular masslevels of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_33	10545499	In this study, we demonstrate that overexpression of sphingosine kinase markedly increased intracellular mass levels of SPP, enhanced proliferation by promoting the G1 to S phase transition, and suppressed serum deprivation- and ceramide-induced apoptosis.	transcription
67698	2	336109	7	NULL	NULL	0	NULL	G1 phase	Process		transition to					S phase	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_33	10545499	In this study, we demonstrate that overexpression of sphingosine kinase markedly increased intracellular mass levels of SPP, enhanced proliferation by promoting the G1 to S phase transition, and suppressed serum deprivation- and ceramide-induced apoptosis.	transcription
67699	3	336109	7	NULL	NULL	NULL	NULL	sphingosine kinase	GP		enhance					proliferation	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_33	10545499	In this study, we demonstrate that overexpression of sphingosine kinase markedly increased intracellular mass levels of SPP, enhanced proliferation by promoting the G1 to S phase transition, and suppressed serum deprivation- and ceramide-induced apoptosis.	transcription
67702	4	336109	7	NULL	NULL	0	NULL	statement 3	Process		occur by					statement 2	Process	promoting			NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_33	10545499	In this study, we demonstrate that overexpression of sphingosine kinase markedly increased intracellular mass levels of SPP, enhanced proliferation by promoting the G1 to S phase transition, and suppressed serum deprivation- and ceramide-induced apoptosis.	transcription
67706	5	336109	7	NULL	NULL	NULL	NULL	sphingosine kinase	GP		suppress					serum deprivation	Process				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_33	10545499	In this study, we demonstrate that overexpression of sphingosine kinase markedly increased intracellular mass levels of SPP, enhanced proliferation by promoting the G1 to S phase transition, and suppressed serum deprivation- and ceramide-induced apoptosis.	transcription
67707	6	336109	7	NULL	NULL	0	NULL	ceramide	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_33	10545499	In this study, we demonstrate that overexpression of sphingosine kinase markedly increased intracellular mass levels of SPP, enhanced proliferation by promoting the G1 to S phase transition, and suppressed serum deprivation- and ceramide-induced apoptosis.	transcription
67708	7	336109	7	NULL	NULL	0	NULL	sphingosine kinase	GP		suppress					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_33	10545499	In this study, we demonstrate that overexpression of sphingosine kinase markedly increased intracellular mass levels of SPP, enhanced proliferation by promoting the G1 to S phase transition, and suppressed serum deprivation- and ceramide-induced apoptosis.	transcription
66617	2	336110	5	NULL	NULL	NULL	NULL	sphingosine kinase	GP	activation of	mediates					statement 1	Process				NULL	hippocampal neurons	NULL	NULL	NULL	NULL	gw60_neuroscience_115_4_1089_s_356	12453482	Overall, our findings provide strong evidence that activation of sphingosine kinase but not NSMase activation or enhanced ceramide synthesis mediated NGF-triggered survival signaling in hippocampal neurons.	transcription
66618	1	336110	5	NULL	NULL	NULL	NULL	survival signaling	Process		is triggerd by					NGF	GP				NULL	hippocampal neurons	NULL	NULL	NULL	NULL	gw60_neuroscience_115_4_1089_s_356	12453482	Overall, our findings provide strong evidence that activation of sphingosine kinase but not NSMase activation or enhanced ceramide synthesis mediated NGF-triggered survival signaling in hippocampal neurons.	transcription
66619	3	336110	5	NULL	NULL	0	NULL	NSMase	GP	activation of	does not mediate					statement 1	Process				NULL	hippocampal neurons	0	NULL	NULL	NULL	gw60_neuroscience_115_4_1089_s_356	12453482	Overall, our findings provide strong evidence that activation of sphingosine kinase but not NSMase activation or enhanced ceramide synthesis mediated NGF-triggered survival signaling in hippocampal neurons.	transcription
66620	4	336110	5	NULL	NULL	0	NULL	ceramide	Chemical	enhanced synthesis of	does not mediate					statement 1	Process				NULL	hippocampal neurons	0	NULL	NULL	NULL	gw60_neuroscience_115_4_1089_s_356	12453482	Overall, our findings provide strong evidence that activation of sphingosine kinase but not NSMase activation or enhanced ceramide synthesis mediated NGF-triggered survival signaling in hippocampal neurons.	transcription
67710	1	336110	7	NULL	NULL	0	NULL	NGF	GP		trigger					survival signaling	Process				NULL	hippocampal neurons	0	NULL	NULL	NULL	gw60_neuroscience_115_4_1089_s_356	12453482	Overall, our findings provide strong evidence that activation of sphingosine kinase but not NSMase activation or enhanced ceramide synthesis mediated NGF-triggered survival signaling in hippocampal neurons.	transcription
67711	2	336110	7	NULL	NULL	0	NULL	sphingosine kinase	GP	activation of	mediate					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_neuroscience_115_4_1089_s_356	12453482	Overall, our findings provide strong evidence that activation of sphingosine kinase but not NSMase activation or enhanced ceramide synthesis mediated NGF-triggered survival signaling in hippocampal neurons.	transcription
67712	3	336110	7	NULL	NULL	0	NULL	NSMase	GP	activation of	does not mediate					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_neuroscience_115_4_1089_s_356	12453482	Overall, our findings provide strong evidence that activation of sphingosine kinase but not NSMase activation or enhanced ceramide synthesis mediated NGF-triggered survival signaling in hippocampal neurons.	transcription
67713	4	336110	7	NULL	NULL	0	NULL	ceramide	Chemical	enhanced synthesis of	mediate					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_neuroscience_115_4_1089_s_356	12453482	Overall, our findings provide strong evidence that activation of sphingosine kinase but not NSMase activation or enhanced ceramide synthesis mediated NGF-triggered survival signaling in hippocampal neurons.	transcription
66621	1	336111	5	NULL	NULL	0	NULL	p42-ERK1/p44-ERK2	GP	basal activity of	is reduced by		gradually			ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_6	9415703	Characterization of the mitogen-activated protein kinase (MAPK) cascade in these responses revealed a further functional disparity between the two lipids: basal p42-ERK1/p44-ERK2 activity was gradually reduced by ceramide but immediately and completely suppressed by sphingosine.	transcription
66622	2	336111	5	NULL	NULL	0	NULL	p42-ERK1/p44-ERK2	GP	basal activity of	suppressed by		immediately;;completely			sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_6	9415703	Characterization of the mitogen-activated protein kinase (MAPK) cascade in these responses revealed a further functional disparity between the two lipids: basal p42-ERK1/p44-ERK2 activity was gradually reduced by ceramide but immediately and completely suppressed by sphingosine.	transcription
67714	1	336111	7	NULL	NULL	0	NULL	ceramide	Chemical		reduce					basal p42-ERK1/p44-ERK2 activity	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_6	9415703	Characterization of the mitogen-activated protein kinase (MAPK) cascade in these responses revealed a further functional disparity between the two lipids: basal p42-ERK1/p44-ERK2 activity was gradually reduced by ceramide but immediately and completely suppressed by sphingosine.	transcription
67715	2	336111	7	NULL	NULL	0	NULL	sphingosine	Chemical		suppress		completely			basal p42-ERK1/p44-ERK2 activity	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_6	9415703	Characterization of the mitogen-activated protein kinase (MAPK) cascade in these responses revealed a further functional disparity between the two lipids: basal p42-ERK1/p44-ERK2 activity was gradually reduced by ceramide but immediately and completely suppressed by sphingosine.	transcription
66623	1	336112	5	NULL	NULL	0	NULL	lipid	Chemical		increases		sharply			p38-RK	GP	activity of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_8	9415703	Both lipids sharply increased p38-RK activity; selective pharmacological inhibition of p38-RK by the pyridinyl imidazole SB-203580 failed to mitigate the cytotoxicity associated with either ceramide or sphingosine, suggesting that p38-RK is not essential for lipid-induced apoptosis.	transcription
66624	2	336112	5	NULL	NULL	NULL	NULL	p38-RK	GP		is inhibited by		selective;;pharmacological			pyridinyl imidazole SB-203580	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_8	9415703	Both lipids sharply increased p38-RK activity; selective pharmacological inhibition of p38-RK by the pyridinyl imidazole SB-203580 failed to mitigate the cytotoxicity associated with either ceramide or sphingosine, suggesting that p38-RK is not essential for lipid-induced apoptosis.	transcription
66627	3	336112	5	NULL	NULL	0	NULL	cytotoxicity	Process		is associated with					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_8	9415703	Both lipids sharply increased p38-RK activity; selective pharmacological inhibition of p38-RK by the pyridinyl imidazole SB-203580 failed to mitigate the cytotoxicity associated with either ceramide or sphingosine, suggesting that p38-RK is not essential for lipid-induced apoptosis.	transcription
66628	4	336112	5	NULL	NULL	0	NULL	cytotoxicity	Process		is associated with					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_8	9415703	Both lipids sharply increased p38-RK activity; selective pharmacological inhibition of p38-RK by the pyridinyl imidazole SB-203580 failed to mitigate the cytotoxicity associated with either ceramide or sphingosine, suggesting that p38-RK is not essential for lipid-induced apoptosis.	transcription
66629	5	336112	5	NULL	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_8	9415703	Both lipids sharply increased p38-RK activity; selective pharmacological inhibition of p38-RK by the pyridinyl imidazole SB-203580 failed to mitigate the cytotoxicity associated with either ceramide or sphingosine, suggesting that p38-RK is not essential for lipid-induced apoptosis.	transcription
66630	6	336112	5	NULL	NULL	0	NULL	statement 2	Process		fails to mitigate					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_8	9415703	Both lipids sharply increased p38-RK activity; selective pharmacological inhibition of p38-RK by the pyridinyl imidazole SB-203580 failed to mitigate the cytotoxicity associated with either ceramide or sphingosine, suggesting that p38-RK is not essential for lipid-induced apoptosis.	transcription
66631	7	336112	5	NULL	NULL	0	NULL	apoptosis	Process		is induced by					lipid	Chemical				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_8	9415703	Both lipids sharply increased p38-RK activity; selective pharmacological inhibition of p38-RK by the pyridinyl imidazole SB-203580 failed to mitigate the cytotoxicity associated with either ceramide or sphingosine, suggesting that p38-RK is not essential for lipid-induced apoptosis.	transcription
66632	8	336112	5	NULL	NULL	0	NULL	p38-RK	GP		is not essential for					statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_8	9415703	Both lipids sharply increased p38-RK activity; selective pharmacological inhibition of p38-RK by the pyridinyl imidazole SB-203580 failed to mitigate the cytotoxicity associated with either ceramide or sphingosine, suggesting that p38-RK is not essential for lipid-induced apoptosis.	transcription
66633	9	336112	5	NULL	NULL	NULL	NULL	statement 6	Process		suggest					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_8	9415703	Both lipids sharply increased p38-RK activity; selective pharmacological inhibition of p38-RK by the pyridinyl imidazole SB-203580 failed to mitigate the cytotoxicity associated with either ceramide or sphingosine, suggesting that p38-RK is not essential for lipid-induced apoptosis.	transcription
67716	1	336112	7	NULL	NULL	NULL	NULL	SB-203580	Chemical		inhibit		selectively;;pharmacological			p38-RK	GP				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_8	9415703	Both lipids sharply increased p38-RK activity; selective pharmacological inhibition of p38-RK by the pyridinyl imidazole SB-203580 failed to mitigate the cytotoxicity associated with either ceramide or sphingosine, suggesting that p38-RK is not essential for lipid-induced apoptosis.	transcription
67717	2	336112	7	NULL	NULL	0	NULL	cytotoxicity	Process		associated with					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_8	9415703	Both lipids sharply increased p38-RK activity; selective pharmacological inhibition of p38-RK by the pyridinyl imidazole SB-203580 failed to mitigate the cytotoxicity associated with either ceramide or sphingosine, suggesting that p38-RK is not essential for lipid-induced apoptosis.	transcription
67718	3	336112	7	NULL	NULL	0	NULL	cytotoxicity	Process		associated with					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_8	9415703	Both lipids sharply increased p38-RK activity; selective pharmacological inhibition of p38-RK by the pyridinyl imidazole SB-203580 failed to mitigate the cytotoxicity associated with either ceramide or sphingosine, suggesting that p38-RK is not essential for lipid-induced apoptosis.	transcription
67719	4	336112	7	NULL	NULL	0	NULL	statement 1	Process		failed to mitigate					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_8	9415703	Both lipids sharply increased p38-RK activity; selective pharmacological inhibition of p38-RK by the pyridinyl imidazole SB-203580 failed to mitigate the cytotoxicity associated with either ceramide or sphingosine, suggesting that p38-RK is not essential for lipid-induced apoptosis.	transcription
67720	5	336112	7	NULL	NULL	0	NULL	statement 1	Process		failed to mitigate					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_8	9415703	Both lipids sharply increased p38-RK activity; selective pharmacological inhibition of p38-RK by the pyridinyl imidazole SB-203580 failed to mitigate the cytotoxicity associated with either ceramide or sphingosine, suggesting that p38-RK is not essential for lipid-induced apoptosis.	transcription
67721	6	336112	7	NULL	NULL	0	NULL	lipid	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_8	9415703	Both lipids sharply increased p38-RK activity; selective pharmacological inhibition of p38-RK by the pyridinyl imidazole SB-203580 failed to mitigate the cytotoxicity associated with either ceramide or sphingosine, suggesting that p38-RK is not essential for lipid-induced apoptosis.	transcription
67722	7	336112	7	NULL	NULL	0	NULL	p38-RK	GP		is not essential for					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_8	9415703	Both lipids sharply increased p38-RK activity; selective pharmacological inhibition of p38-RK by the pyridinyl imidazole SB-203580 failed to mitigate the cytotoxicity associated with either ceramide or sphingosine, suggesting that p38-RK is not essential for lipid-induced apoptosis.	transcription
67723	8	336112	7	NULL	NULL	0	NULL	statement 4	Process		suggest					statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_8	9415703	Both lipids sharply increased p38-RK activity; selective pharmacological inhibition of p38-RK by the pyridinyl imidazole SB-203580 failed to mitigate the cytotoxicity associated with either ceramide or sphingosine, suggesting that p38-RK is not essential for lipid-induced apoptosis.	transcription
67724	9	336112	7	NULL	NULL	0	NULL	statement 5	Process		suggest					statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_8	9415703	Both lipids sharply increased p38-RK activity; selective pharmacological inhibition of p38-RK by the pyridinyl imidazole SB-203580 failed to mitigate the cytotoxicity associated with either ceramide or sphingosine, suggesting that p38-RK is not essential for lipid-induced apoptosis.	transcription
67726	10	336112	7	NULL	NULL	0	NULL	SB-203580	Chemical		is a type of					pyridinyl imidazole	Chemical				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_8	9415703	Both lipids sharply increased p38-RK activity; selective pharmacological inhibition of p38-RK by the pyridinyl imidazole SB-203580 failed to mitigate the cytotoxicity associated with either ceramide or sphingosine, suggesting that p38-RK is not essential for lipid-induced apoptosis.	transcription
66635	1	336113	5	NULL	NULL	0	NULL	lipids	Chemical	lethal actions of	entail alterations in		reciprocal;;coordinated			SAPK	GP	activity of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_29	9415703	The results demonstrate that the lethal actions of these lipids entail reciprocal, but coordinated, alterations in SAPK and MAPK activities such that both ceramide and sphingosine stimulate p46-JNK1/p54-JNK2 but suppress p42-ERK1/p44-ERK2, albeit to varying degrees.	transcription
66636	2	336113	5	NULL	NULL	0	NULL	lipids	Chemical	lethal actions of	entail alterations in		reciprocal;;coordinated			MAPK	GP	activity of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_29	9415703	The results demonstrate that the lethal actions of these lipids entail reciprocal, but coordinated, alterations in SAPK and MAPK activities such that both ceramide and sphingosine stimulate p46-JNK1/p54-JNK2 but suppress p42-ERK1/p44-ERK2, albeit to varying degrees.	transcription
66637	3	336113	5	NULL	NULL	0	NULL	ceramide	Chemical		stimulates					p46-JNK1/p54-JNK2	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_29	9415703	The results demonstrate that the lethal actions of these lipids entail reciprocal, but coordinated, alterations in SAPK and MAPK activities such that both ceramide and sphingosine stimulate p46-JNK1/p54-JNK2 but suppress p42-ERK1/p44-ERK2, albeit to varying degrees.	transcription
66638	4	336113	5	NULL	NULL	0	NULL	sphingosine	Chemical		stimulates					p46-JNK1/p54-JNK2	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_29	9415703	The results demonstrate that the lethal actions of these lipids entail reciprocal, but coordinated, alterations in SAPK and MAPK activities such that both ceramide and sphingosine stimulate p46-JNK1/p54-JNK2 but suppress p42-ERK1/p44-ERK2, albeit to varying degrees.	transcription
66639	5	336113	5	NULL	NULL	0	NULL	ceramide	Chemical		suppress					p42-ERK1/p44-ERK2	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_29	9415703	The results demonstrate that the lethal actions of these lipids entail reciprocal, but coordinated, alterations in SAPK and MAPK activities such that both ceramide and sphingosine stimulate p46-JNK1/p54-JNK2 but suppress p42-ERK1/p44-ERK2, albeit to varying degrees.	transcription
66640	6	336113	5	NULL	NULL	0	NULL	sphingosine	Chemical		suppress					p42-ERK1/p44-ERK2	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_29	9415703	The results demonstrate that the lethal actions of these lipids entail reciprocal, but coordinated, alterations in SAPK and MAPK activities such that both ceramide and sphingosine stimulate p46-JNK1/p54-JNK2 but suppress p42-ERK1/p44-ERK2, albeit to varying degrees.	transcription
67725	1	336113	7	NULL	NULL	0	NULL	ceramide	Chemical		stimulate					p46-JNK1/p54-JNK2	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_29	9415703	The results demonstrate that the lethal actions of these lipids entail reciprocal, but coordinated, alterations in SAPK and MAPK activities such that both ceramide and sphingosine stimulate p46-JNK1/p54-JNK2 but suppress p42-ERK1/p44-ERK2, albeit to varying degrees.	transcription
67727	2	336113	7	NULL	NULL	0	NULL	sphingosine	Chemical		stimulate					p46-JNK1/p54-JNK2	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_29	9415703	The results demonstrate that the lethal actions of these lipids entail reciprocal, but coordinated, alterations in SAPK and MAPK activities such that both ceramide and sphingosine stimulate p46-JNK1/p54-JNK2 but suppress p42-ERK1/p44-ERK2, albeit to varying degrees.	transcription
67728	3	336113	7	NULL	NULL	0	NULL	ceramide	Chemical		suppress					p42-ERK1/p44-ERK2	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_29	9415703	The results demonstrate that the lethal actions of these lipids entail reciprocal, but coordinated, alterations in SAPK and MAPK activities such that both ceramide and sphingosine stimulate p46-JNK1/p54-JNK2 but suppress p42-ERK1/p44-ERK2, albeit to varying degrees.	transcription
67729	4	336113	7	NULL	NULL	0	NULL	sphingosine	Chemical		suppress					p42-ERK1/p44-ERK2	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_29	9415703	The results demonstrate that the lethal actions of these lipids entail reciprocal, but coordinated, alterations in SAPK and MAPK activities such that both ceramide and sphingosine stimulate p46-JNK1/p54-JNK2 but suppress p42-ERK1/p44-ERK2, albeit to varying degrees.	transcription
66641	1	336115	5	NULL	NULL	0	NULL	ceramide	Chemical		elicits					p38-RK	GP	complex activation of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_339	9415703	The complex activation of p38-RK elicited by ceramide and sphingosine may therefore represent a consequence, rather than a cause, of lipid-induced apoptosis and possibly constitutes a cytoprotective response to lethal insult.	transcription
66642	2	336115	5	NULL	NULL	0	NULL	sphingosine	Chemical		elicits					p38-RK	GP	complex activation of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_339	9415703	The complex activation of p38-RK elicited by ceramide and sphingosine may therefore represent a consequence, rather than a cause, of lipid-induced apoptosis and possibly constitutes a cytoprotective response to lethal insult.	transcription
66643	3	336115	5	NULL	NULL	0	NULL	apoptosis	Process		is induced by					lipid	Chemical				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_339	9415703	The complex activation of p38-RK elicited by ceramide and sphingosine may therefore represent a consequence, rather than a cause, of lipid-induced apoptosis and possibly constitutes a cytoprotective response to lethal insult.	transcription
66644	4	336115	5	NULL	NULL	0	NULL	statement 3	Process		leads to					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_339	9415703	The complex activation of p38-RK elicited by ceramide and sphingosine may therefore represent a consequence, rather than a cause, of lipid-induced apoptosis and possibly constitutes a cytoprotective response to lethal insult.	transcription
66645	5	336115	5	NULL	NULL	0	NULL	statement 3	Process		leads to					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_339	9415703	The complex activation of p38-RK elicited by ceramide and sphingosine may therefore represent a consequence, rather than a cause, of lipid-induced apoptosis and possibly constitutes a cytoprotective response to lethal insult.	transcription
67730	1	336115	7	NULL	NULL	NULL	NULL	ceramide	Chemical		elicit					p38-RK	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_339	9415703	The complex activation of p38-RK elicited by ceramide and sphingosine may therefore represent a consequence, rather than a cause, of lipid-induced apoptosis and possibly constitutes a cytoprotective response to lethal insult.	transcription
67731	2	336115	7	NULL	NULL	0	NULL	sphingosine	Chemical		elicit					p38-RK	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_339	9415703	The complex activation of p38-RK elicited by ceramide and sphingosine may therefore represent a consequence, rather than a cause, of lipid-induced apoptosis and possibly constitutes a cytoprotective response to lethal insult.	transcription
67732	3	336115	7	NULL	NULL	0	NULL	lipid	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_339	9415703	The complex activation of p38-RK elicited by ceramide and sphingosine may therefore represent a consequence, rather than a cause, of lipid-induced apoptosis and possibly constitutes a cytoprotective response to lethal insult.	transcription
67733	4	336115	7	NULL	NULL	0	NULL	statement 1	Process		represent					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_339	9415703	The complex activation of p38-RK elicited by ceramide and sphingosine may therefore represent a consequence, rather than a cause, of lipid-induced apoptosis and possibly constitutes a cytoprotective response to lethal insult.	transcription
67734	5	336115	7	NULL	NULL	0	NULL	statement 2	Process		represent					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_339	9415703	The complex activation of p38-RK elicited by ceramide and sphingosine may therefore represent a consequence, rather than a cause, of lipid-induced apoptosis and possibly constitutes a cytoprotective response to lethal insult.	transcription
66646	1	336116	5	NULL	NULL	0	NULL	ceramide	Chemical		stimulates		strongly			SAPK	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_346	9415703	In the primary induction of apoptosis, we found that (a) ceramide strongly stimulates SAPK and weakly inhibits MAPK, whereas (b) sphingosine weakly stimulates SAPK but strongly inhibits MAPK.	transcription
66647	2	336116	5	NULL	NULL	0	NULL	ceramide	Chemical		inhibits		weakly			MAPK	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_346	9415703	In the primary induction of apoptosis, we found that (a) ceramide strongly stimulates SAPK and weakly inhibits MAPK, whereas (b) sphingosine weakly stimulates SAPK but strongly inhibits MAPK.	transcription
66648	3	336116	5	NULL	NULL	0	NULL	sphingosine	Chemical		stimulates		weakly			SAPK	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_346	9415703	In the primary induction of apoptosis, we found that (a) ceramide strongly stimulates SAPK and weakly inhibits MAPK, whereas (b) sphingosine weakly stimulates SAPK but strongly inhibits MAPK.	transcription
66649	4	336116	5	NULL	NULL	0	NULL	sphingosine	Chemical		inhibits		strongly			MAPK	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_346	9415703	In the primary induction of apoptosis, we found that (a) ceramide strongly stimulates SAPK and weakly inhibits MAPK, whereas (b) sphingosine weakly stimulates SAPK but strongly inhibits MAPK.	transcription
66650	5	336116	5	NULL	NULL	0	NULL	statement 1	Process		occurs during					apoptosis	Process	primary induction of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_346	9415703	In the primary induction of apoptosis, we found that (a) ceramide strongly stimulates SAPK and weakly inhibits MAPK, whereas (b) sphingosine weakly stimulates SAPK but strongly inhibits MAPK.	transcription
66651	6	336116	5	NULL	NULL	0	NULL	statement 2	Process		occurs during					apoptosis	Process	primary induction of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_346	9415703	In the primary induction of apoptosis, we found that (a) ceramide strongly stimulates SAPK and weakly inhibits MAPK, whereas (b) sphingosine weakly stimulates SAPK but strongly inhibits MAPK.	transcription
66652	7	336116	5	NULL	NULL	0	NULL	statement 3	Process		occurs during					apoptosis	Process	primary induction of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_346	9415703	In the primary induction of apoptosis, we found that (a) ceramide strongly stimulates SAPK and weakly inhibits MAPK, whereas (b) sphingosine weakly stimulates SAPK but strongly inhibits MAPK.	transcription
66653	8	336116	5	NULL	NULL	0	NULL	statement 4	Process		occurs during					apoptosis	Process	primary induction of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_346	9415703	In the primary induction of apoptosis, we found that (a) ceramide strongly stimulates SAPK and weakly inhibits MAPK, whereas (b) sphingosine weakly stimulates SAPK but strongly inhibits MAPK.	transcription
67735	1	336116	7	NULL	NULL	0	NULL	ceramide	Chemical		stimulate		strongly			SAPK	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_346	9415703	In the primary induction of apoptosis, we found that (a) ceramide strongly stimulates SAPK and weakly inhibits MAPK, whereas (b) sphingosine weakly stimulates SAPK but strongly inhibits MAPK.	transcription
67736	2	336116	7	NULL	NULL	0	NULL	ceramide	Chemical		inhibit		weakly			MAPK	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_346	9415703	In the primary induction of apoptosis, we found that (a) ceramide strongly stimulates SAPK and weakly inhibits MAPK, whereas (b) sphingosine weakly stimulates SAPK but strongly inhibits MAPK.	transcription
67737	3	336116	7	NULL	NULL	0	NULL	sphingosine	Chemical		stimulate		weakly			MAPK	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_346	9415703	In the primary induction of apoptosis, we found that (a) ceramide strongly stimulates SAPK and weakly inhibits MAPK, whereas (b) sphingosine weakly stimulates SAPK but strongly inhibits MAPK.	transcription
67738	4	336116	7	NULL	NULL	0	NULL	sphingosine	Chemical		inhibit		strongly			MAPK	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_346	9415703	In the primary induction of apoptosis, we found that (a) ceramide strongly stimulates SAPK and weakly inhibits MAPK, whereas (b) sphingosine weakly stimulates SAPK but strongly inhibits MAPK.	transcription
67739	5	336116	7	NULL	NULL	0	NULL	statement 1	Process		occur during					apoptosis	Process	primary induction of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_346	9415703	In the primary induction of apoptosis, we found that (a) ceramide strongly stimulates SAPK and weakly inhibits MAPK, whereas (b) sphingosine weakly stimulates SAPK but strongly inhibits MAPK.	transcription
67740	6	336116	7	NULL	NULL	0	NULL	statement 2	Process		occur during					apoptosis	Process	primary induction of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_346	9415703	In the primary induction of apoptosis, we found that (a) ceramide strongly stimulates SAPK and weakly inhibits MAPK, whereas (b) sphingosine weakly stimulates SAPK but strongly inhibits MAPK.	transcription
67741	7	336116	7	NULL	NULL	0	NULL	statement 3	Process		occur during					apoptosis	Process	primary induction of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_346	9415703	In the primary induction of apoptosis, we found that (a) ceramide strongly stimulates SAPK and weakly inhibits MAPK, whereas (b) sphingosine weakly stimulates SAPK but strongly inhibits MAPK.	transcription
67742	8	336116	7	NULL	NULL	0	NULL	statement 4	Process		occur during					apoptosis	Process	primary induction of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_346	9415703	In the primary induction of apoptosis, we found that (a) ceramide strongly stimulates SAPK and weakly inhibits MAPK, whereas (b) sphingosine weakly stimulates SAPK but strongly inhibits MAPK.	transcription
66654	1	336117	5	NULL	NULL	0	NULL	LPS	Chemical		induce					ceramide	Chemical	level of			NULL	old mice	0	NULL	NULL	NULL	gw60_jbiolchem_277_34_30784_s_5	12072440	Furthermore, the results show that LPS-induced ceramide levels from the old mice are significantly higher than those of young mice, whereas there is no age-related difference in concentration of its down stream metabolite, sphingosine.	transcription
66655	2	336117	5	NULL	NULL	0	NULL	LPS	Chemical		induce					ceramide	Chemical	level of			NULL	young mice	0	NULL	NULL	NULL	gw60_jbiolchem_277_34_30784_s_5	12072440	Furthermore, the results show that LPS-induced ceramide levels from the old mice are significantly higher than those of young mice, whereas there is no age-related difference in concentration of its down stream metabolite, sphingosine.	transcription
66656	3	336117	5	NULL	NULL	0	NULL	statement 1	Process		is higher than		significantly			statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_34_30784_s_5	12072440	Furthermore, the results show that LPS-induced ceramide levels from the old mice are significantly higher than those of young mice, whereas there is no age-related difference in concentration of its down stream metabolite, sphingosine.	transcription
67743	1	336117	7	NULL	NULL	0	NULL	LPS	Chemical		induce					ceramide	Chemical	levels of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_34_30784_s_5	12072440	Furthermore, the results show that LPS-induced ceramide levels from the old mice are significantly higher than those of young mice, whereas there is no age-related difference in concentration of its down stream metabolite, sphingosine.	transcription
66739	1	336118	5	NULL	NULL	0	NULL	TNF-alpha	GP		stimulates					GTPCH	GP	expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_33	11815603	As TNF-alpha stimulates GTPCH expression via a ceramide-independent pathway ( 12) and increases SPP levels ( 17-19), it was of interest to investigate the role of sphingosine kinase and SPP in the regulation of GTPCH and BH4 biosynthesis.	transcription
66740	2	336118	5	NULL	NULL	0	NULL	statement 1	Process		via					ceramide-independent pathway	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_33	11815603	As TNF-alpha stimulates GTPCH expression via a ceramide-independent pathway ( 12) and increases SPP levels ( 17-19), it was of interest to investigate the role of sphingosine kinase and SPP in the regulation of GTPCH and BH4 biosynthesis.	transcription
66741	3	336118	5	NULL	NULL	0	NULL	statement 1	Process		increases					SPP	Chemical	level of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_33	11815603	As TNF-alpha stimulates GTPCH expression via a ceramide-independent pathway ( 12) and increases SPP levels ( 17-19), it was of interest to investigate the role of sphingosine kinase and SPP in the regulation of GTPCH and BH4 biosynthesis.	transcription
66742	4	336118	5	NULL	NULL	NULL	NULL	sphingosine kinase	GP		regulates		potentially			GTPCH	GP	biosynthesis of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_33	11815603	As TNF-alpha stimulates GTPCH expression via a ceramide-independent pathway ( 12) and increases SPP levels ( 17-19), it was of interest to investigate the role of sphingosine kinase and SPP in the regulation of GTPCH and BH4 biosynthesis.	transcription
66743	5	336118	5	NULL	NULL	NULL	NULL	sphingosine kinase	GP		regulates		potentially			BH4	Chemical	biosynthesis of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_33	11815603	As TNF-alpha stimulates GTPCH expression via a ceramide-independent pathway ( 12) and increases SPP levels ( 17-19), it was of interest to investigate the role of sphingosine kinase and SPP in the regulation of GTPCH and BH4 biosynthesis.	transcription
66744	6	336118	5	NULL	NULL	0	NULL	SPP	Chemical		regulates		potentially			GTPCH	GP	biosynthesis of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_33	11815603	As TNF-alpha stimulates GTPCH expression via a ceramide-independent pathway ( 12) and increases SPP levels ( 17-19), it was of interest to investigate the role of sphingosine kinase and SPP in the regulation of GTPCH and BH4 biosynthesis.	transcription
66745	7	336118	5	NULL	NULL	0	NULL	SPP	Chemical		regulates		potentially			BH4	Chemical	biosynthesis of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_33	11815603	As TNF-alpha stimulates GTPCH expression via a ceramide-independent pathway ( 12) and increases SPP levels ( 17-19), it was of interest to investigate the role of sphingosine kinase and SPP in the regulation of GTPCH and BH4 biosynthesis.	transcription
67744	1	336118	7	NULL	NULL	0	NULL	TNF-alpha	GP		stimulate					GTPCH	GP	expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_33	11815603	As TNF-alpha stimulates GTPCH expression via a ceramide-independent pathway ( 12) and increases SPP levels ( 17-19), it was of interest to investigate the role of sphingosine kinase and SPP in the regulation of GTPCH and BH4 biosynthesis.	transcription
67745	2	336118	7	NULL	NULL	0	NULL	statement 1	Process		via					ceramide-independent pathway	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_33	11815603	As TNF-alpha stimulates GTPCH expression via a ceramide-independent pathway ( 12) and increases SPP levels ( 17-19), it was of interest to investigate the role of sphingosine kinase and SPP in the regulation of GTPCH and BH4 biosynthesis.	transcription
67746	3	336118	7	NULL	NULL	0	NULL	statement 1	Process		increase					SPP 	Chemical	levels of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_33	11815603	As TNF-alpha stimulates GTPCH expression via a ceramide-independent pathway ( 12) and increases SPP levels ( 17-19), it was of interest to investigate the role of sphingosine kinase and SPP in the regulation of GTPCH and BH4 biosynthesis.	transcription
66756	1	336119	5	NULL	NULL	NULL	NULL	long chain ceramide	Chemical	generation of	in response to					C6-ceramide	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_12960_s_163	11815611	Therefore, these results further demonstrate that the generation of endogenous long chain ceramide formation in response to C6-ceramide is not via the activation of the  de novo pathway but involves the recycling of the sphingosine backbone following deacylation and reacylation, a process inhibited by FB1.	transcription
66757	2	336119	5	NULL	NULL	NULL	NULL	statement 1	Process		is not via					de novo pathway	Process	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_12960_s_163	11815611	Therefore, these results further demonstrate that the generation of endogenous long chain ceramide formation in response to C6-ceramide is not via the activation of the  de novo pathway but involves the recycling of the sphingosine backbone following deacylation and reacylation, a process inhibited by FB1.	transcription
66758	3	336119	5	NULL	NULL	0	NULL	statement 1	Process		involves					sphingosine backbone	Chemical	recycling of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12960_s_163	11815611	Therefore, these results further demonstrate that the generation of endogenous long chain ceramide formation in response to C6-ceramide is not via the activation of the  de novo pathway but involves the recycling of the sphingosine backbone following deacylation and reacylation, a process inhibited by FB1.	transcription
66759	4	336119	5	NULL	NULL	0	NULL	statement 3	Process		followed by					ceramide	Chemical	deacylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12960_s_163	11815611	Therefore, these results further demonstrate that the generation of endogenous long chain ceramide formation in response to C6-ceramide is not via the activation of the  de novo pathway but involves the recycling of the sphingosine backbone following deacylation and reacylation, a process inhibited by FB1.	transcription
66760	5	336119	5	NULL	NULL	0	NULL	statement 3	Process		followed by					ceramide	Chemical	reacylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12960_s_163	11815611	Therefore, these results further demonstrate that the generation of endogenous long chain ceramide formation in response to C6-ceramide is not via the activation of the  de novo pathway but involves the recycling of the sphingosine backbone following deacylation and reacylation, a process inhibited by FB1.	transcription
66761	6	336119	5	NULL	NULL	0	NULL	FB1	Chemical		inhibits					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12960_s_163	11815611	Therefore, these results further demonstrate that the generation of endogenous long chain ceramide formation in response to C6-ceramide is not via the activation of the  de novo pathway but involves the recycling of the sphingosine backbone following deacylation and reacylation, a process inhibited by FB1.	transcription
67747	1	336119	7	NULL	NULL	0	NULL	 long chain ceramide	Chemical	formation of;;endogenous	in response to					C6-ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12960_s_163	11815611	Therefore, these results further demonstrate that the generation of endogenous long chain ceramide formation in response to C6-ceramide is not via the activation of the  de novo pathway but involves the recycling of the sphingosine backbone following deacylation and reacylation, a process inhibited by FB1.	transcription
67748	2	336119	7	NULL	NULL	0	NULL	statement 1	Process		not via					de novo pathway	Process	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12960_s_163	11815611	Therefore, these results further demonstrate that the generation of endogenous long chain ceramide formation in response to C6-ceramide is not via the activation of the  de novo pathway but involves the recycling of the sphingosine backbone following deacylation and reacylation, a process inhibited by FB1.	transcription
67749	3	336119	7	NULL	NULL	NULL	NULL	statement 1	Process		involves					sphingosine backbone	Chemical	recycling of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_12960_s_163	11815611	Therefore, these results further demonstrate that the generation of endogenous long chain ceramide formation in response to C6-ceramide is not via the activation of the  de novo pathway but involves the recycling of the sphingosine backbone following deacylation and reacylation, a process inhibited by FB1.	transcription
67750	4	336119	7	NULL	NULL	0	NULL	FB1	Chemical		inhibit					sphingosine backbone	Chemical	deacylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12960_s_163	11815611	Therefore, these results further demonstrate that the generation of endogenous long chain ceramide formation in response to C6-ceramide is not via the activation of the  de novo pathway but involves the recycling of the sphingosine backbone following deacylation and reacylation, a process inhibited by FB1.	transcription
67751	5	336119	7	NULL	NULL	0	NULL	FB1	Chemical		inhibit					sphingosine backbone	Chemical	reacylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12960_s_163	11815611	Therefore, these results further demonstrate that the generation of endogenous long chain ceramide formation in response to C6-ceramide is not via the activation of the  de novo pathway but involves the recycling of the sphingosine backbone following deacylation and reacylation, a process inhibited by FB1.	transcription
66762	1	336120	5	NULL	NULL	0	NULL	MFs	Cell	human	undergoes					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_40_37323_s_117	12138095	Indeed, both ceramide and sphingosine induced apoptosis of human hMFs, as shown by increased nuclei fragmentation (Fig.  3 A), DNA laddering (Fig.  3 B), and decreased cell viability (Fig.  3 C).	transcription
66763	2	336120	5	NULL	NULL	0	NULL	ceramide	Chemical		induce					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_40_37323_s_117	12138095	Indeed, both ceramide and sphingosine induced apoptosis of human hMFs, as shown by increased nuclei fragmentation (Fig.  3 A), DNA laddering (Fig.  3 B), and decreased cell viability (Fig.  3 C).	transcription
66764	3	336120	5	NULL	NULL	0	NULL	sphingosine	Chemical		induce					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_40_37323_s_117	12138095	Indeed, both ceramide and sphingosine induced apoptosis of human hMFs, as shown by increased nuclei fragmentation (Fig.  3 A), DNA laddering (Fig.  3 B), and decreased cell viability (Fig.  3 C).	transcription
67752	1	336120	7	NULL	NULL	NULL	NULL	ceramide	Chemical		induce					apoptosis	Process				NULL	human hMFs	NULL	NULL	NULL	NULL	gw60_jbiolchem_277_40_37323_s_117	12138095	Indeed, both ceramide and sphingosine induced apoptosis of human hMFs, as shown by increased nuclei fragmentation (Fig.  3 A), DNA laddering (Fig.  3 B), and decreased cell viability (Fig.  3 C).	transcription
67753	2	336120	7	NULL	NULL	0	NULL	sphingosine	Chemical		induce					apoptosis	Process				NULL	human hMFs	0	NULL	NULL	NULL	gw60_jbiolchem_277_40_37323_s_117	12138095	Indeed, both ceramide and sphingosine induced apoptosis of human hMFs, as shown by increased nuclei fragmentation (Fig.  3 A), DNA laddering (Fig.  3 B), and decreased cell viability (Fig.  3 C).	transcription
66765	1	336121	5	NULL	NULL	0	NULL	ceramide	Chemical	apoptotic effects of	requires					S1P	Chemical	high micromolar concentrations of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_40_37323_s_119	12138095	As shown in Fig.  3 C, apoptotic effects of ceramide and sphingosine required high micromolar concentrations like S1P, arguing against an apoptotic effect of S1P related to metabolite conversion.	transcription
66766	2	336121	5	NULL	NULL	0	NULL	sphingosine	Chemical	apoptotic effects of	requires					S1P	Chemical	high micromolar concentrations of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_40_37323_s_119	12138095	As shown in Fig.  3 C, apoptotic effects of ceramide and sphingosine required high micromolar concentrations like S1P, arguing against an apoptotic effect of S1P related to metabolite conversion.	transcription
67754	1	336121	7	NULL	NULL	0	NULL	ceramide	Chemical	apoptotic effects of 	require					S1P	Chemical	high concentration of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_40_37323_s_119	12138095	As shown in Fig.  3 C, apoptotic effects of ceramide and sphingosine required high micromolar concentrations like S1P, arguing against an apoptotic effect of S1P related to metabolite conversion.	transcription
67755	2	336121	7	NULL	NULL	0	NULL	sphingosine	Chemical	apoptotic effects of 	require					S1P	Chemical	high concentration of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_40_37323_s_119	12138095	As shown in Fig.  3 C, apoptotic effects of ceramide and sphingosine required high micromolar concentrations like S1P, arguing against an apoptotic effect of S1P related to metabolite conversion.	transcription
66767	1	336122	5	NULL	NULL	0	NULL	DGKgamma	GP	human	catalyzes					diacylglycerol	Chemical	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23294_s_126	11956206	In comparison with human DGKgamma, bacterial DGK, and human SPK1, these lysates were enriched in specific ATP-dependent ceramide-phosphorylating activity and did not significantly catalyze the phosphorylation of diacylglycerol or sphingosine (Fig.  2 A).	transcription
66768	2	336122	5	NULL	NULL	0	NULL	DGKgamma	GP	human	catalyzes					sphingosine	Chemical	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23294_s_126	11956206	In comparison with human DGKgamma, bacterial DGK, and human SPK1, these lysates were enriched in specific ATP-dependent ceramide-phosphorylating activity and did not significantly catalyze the phosphorylation of diacylglycerol or sphingosine (Fig.  2 A).	transcription
66769	3	336122	5	NULL	NULL	0	NULL	DGK	GP	bacterial	catalyzes					diacylglycerol	Chemical	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23294_s_126	11956206	In comparison with human DGKgamma, bacterial DGK, and human SPK1, these lysates were enriched in specific ATP-dependent ceramide-phosphorylating activity and did not significantly catalyze the phosphorylation of diacylglycerol or sphingosine (Fig.  2 A).	transcription
66770	4	336122	5	NULL	NULL	0	NULL	DGK	GP	bacterial	catalyzes					sphingosine	Chemical	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23294_s_126	11956206	In comparison with human DGKgamma, bacterial DGK, and human SPK1, these lysates were enriched in specific ATP-dependent ceramide-phosphorylating activity and did not significantly catalyze the phosphorylation of diacylglycerol or sphingosine (Fig.  2 A).	transcription
66771	5	336122	5	NULL	NULL	0	NULL	SPK1	GP	human	catalyzes					diacylglycerol	Chemical	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23294_s_126	11956206	In comparison with human DGKgamma, bacterial DGK, and human SPK1, these lysates were enriched in specific ATP-dependent ceramide-phosphorylating activity and did not significantly catalyze the phosphorylation of diacylglycerol or sphingosine (Fig.  2 A).	transcription
66772	6	336122	5	NULL	NULL	0	NULL	SPK1	GP	human	catalyzes					sphingosine	Chemical	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_26_23294_s_126	11956206	In comparison with human DGKgamma, bacterial DGK, and human SPK1, these lysates were enriched in specific ATP-dependent ceramide-phosphorylating activity and did not significantly catalyze the phosphorylation of diacylglycerol or sphingosine (Fig.  2 A).	transcription
66773	1	336123	5	NULL	NULL	0	NULL	(CHO)1 cells	Cell		is					Chinese hamster ovary 1 cells	Cell				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4046_s_24	11058589	Here we show that short chain ceramide analogs and sphingosine inhibit Na+/Ca2+ exchange activity in transfected Chinese hamster ovary (CHO)1 cells expressing the bovine or canine cardiac Na+/Ca2+ exchangers.	transcription
66776	2	336123	5	NULL	NULL	0	NULL	short chain ceramide analogs	Chemical		inhibits					Na+/Ca2+ exchange activity	Process				NULL	transfected Chinese hamster ovary (CHO)1 cells expressing bovine cardiac Na+/Ca2+ exchangers	0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4046_s_24	11058589	Here we show that short chain ceramide analogs and sphingosine inhibit Na+/Ca2+ exchange activity in transfected Chinese hamster ovary (CHO)1 cells expressing the bovine or canine cardiac Na+/Ca2+ exchangers.	transcription
66777	3	336123	5	NULL	NULL	0	NULL	short chain ceramide analogs	Chemical		inhibits					Na+/Ca2+ exchange activity	Process				NULL	transfected Chinese hamster ovary (CHO)1 cells expressing canine cardiac Na+/Ca2+ exchangers	0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4046_s_24	11058589	Here we show that short chain ceramide analogs and sphingosine inhibit Na+/Ca2+ exchange activity in transfected Chinese hamster ovary (CHO)1 cells expressing the bovine or canine cardiac Na+/Ca2+ exchangers.	transcription
66778	4	336123	5	NULL	NULL	0	NULL	sphingosine	Chemical		inhibits					Na+/Ca2+ exchange activity	Process				NULL	transfected Chinese hamster ovary (CHO)1 cells expressing bovine cardiac Na+/Ca2+ exchangers	0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4046_s_24	11058589	Here we show that short chain ceramide analogs and sphingosine inhibit Na+/Ca2+ exchange activity in transfected Chinese hamster ovary (CHO)1 cells expressing the bovine or canine cardiac Na+/Ca2+ exchangers.	transcription
66779	5	336123	5	NULL	NULL	0	NULL	sphingosine	Chemical		inhibits					Na+/Ca2+ exchange activity	Process				NULL	transfected Chinese hamster ovary (CHO)1 cells expressing canine cardiac Na+/Ca2+ exchangers	0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4046_s_24	11058589	Here we show that short chain ceramide analogs and sphingosine inhibit Na+/Ca2+ exchange activity in transfected Chinese hamster ovary (CHO)1 cells expressing the bovine or canine cardiac Na+/Ca2+ exchangers.	transcription
67759	1	336123	7	NULL	NULL	0	NULL	short chain ceramide analogs	Chemical		inhibit					Na+/Ca2+ exchange activity 	Process				NULL	(CHO)1 cells expressing the bovine cardiac Na+/Ca2+ exchangers	0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4046_s_24	11058589	Here we show that short chain ceramide analogs and sphingosine inhibit Na+/Ca2+ exchange activity in transfected Chinese hamster ovary (CHO)1 cells expressing the bovine or canine cardiac Na+/Ca2+ exchangers.	transcription
67760	2	336123	7	NULL	NULL	0	NULL	short chain ceramide analogs	Chemical		inhibit					Na+/Ca2+ exchange activity	Process				NULL	(CHO)1 cells expressing the canine cardiac Na+/Ca2+ exchangers	0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4046_s_24	11058589	Here we show that short chain ceramide analogs and sphingosine inhibit Na+/Ca2+ exchange activity in transfected Chinese hamster ovary (CHO)1 cells expressing the bovine or canine cardiac Na+/Ca2+ exchangers.	transcription
67761	3	336123	7	NULL	NULL	0	NULL	sphingosine	Chemical		inhibit					Na+/Ca2+ exchange activity	Process				NULL	(CHO)1 cells expressing the bovine cardiac Na+/Ca2+ exchangers	0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4046_s_24	11058589	Here we show that short chain ceramide analogs and sphingosine inhibit Na+/Ca2+ exchange activity in transfected Chinese hamster ovary (CHO)1 cells expressing the bovine or canine cardiac Na+/Ca2+ exchangers.	transcription
67762	4	336123	7	NULL	NULL	0	NULL	sphingosine	Chemical		inhibit					Na+/Ca2+ exchange activity 	Process				NULL	(CHO)1 cells expressing the canine cardiac Na+/Ca2+ exchangers	0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4046_s_24	11058589	Here we show that short chain ceramide analogs and sphingosine inhibit Na+/Ca2+ exchange activity in transfected Chinese hamster ovary (CHO)1 cells expressing the bovine or canine cardiac Na+/Ca2+ exchangers.	transcription
67763	5	336123	7	NULL	NULL	0	NULL	(CHO)1 cells	Cell		is					Chinese hamster ovary cells	Cell				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_6_4046_s_24	11058589	Here we show that short chain ceramide analogs and sphingosine inhibit Na+/Ca2+ exchange activity in transfected Chinese hamster ovary (CHO)1 cells expressing the bovine or canine cardiac Na+/Ca2+ exchangers.	transcription
66780	1	336124	5	NULL	NULL	0	NULL	C2-ceramide	Chemical	treatment;;exogenous	leads to					cell death	Process				NULL	LM cells	0	NULL	NULL	NULL	gw60_jbiolchem_276_29_27129_s_5	11369765	Treatment with exogenous C2-ceramide and sphingosine led to cell death in both LM and LME6, and treatment of the LME6 cells with MNNG resulted in a transient increase in intracellular ceramide of ~50% over a period of 3 h.	transcription
66781	2	336124	5	NULL	NULL	0	NULL	C2-ceramide	Chemical	treatment;;exogenous	leads to					cell death	Process				NULL	LME6 cells	0	NULL	NULL	NULL	gw60_jbiolchem_276_29_27129_s_5	11369765	Treatment with exogenous C2-ceramide and sphingosine led to cell death in both LM and LME6, and treatment of the LME6 cells with MNNG resulted in a transient increase in intracellular ceramide of ~50% over a period of 3 h.	transcription
66782	3	336124	5	NULL	NULL	0	NULL	sphingosine	Chemical	treatment	leads to					cell death	Process				NULL	LM cells	0	NULL	NULL	NULL	gw60_jbiolchem_276_29_27129_s_5	11369765	Treatment with exogenous C2-ceramide and sphingosine led to cell death in both LM and LME6, and treatment of the LME6 cells with MNNG resulted in a transient increase in intracellular ceramide of ~50% over a period of 3 h.	transcription
66783	4	336124	5	NULL	NULL	0	NULL	sphingosine	Chemical	treatment	leads to					cell death	Process				NULL	LME6 cells	0	NULL	NULL	NULL	gw60_jbiolchem_276_29_27129_s_5	11369765	Treatment with exogenous C2-ceramide and sphingosine led to cell death in both LM and LME6, and treatment of the LME6 cells with MNNG resulted in a transient increase in intracellular ceramide of ~50% over a period of 3 h.	transcription
66784	5	336124	5	NULL	NULL	0	NULL	MNNG	Chemical	treatment	results in					ceramide	Chemical	transient increase in;;intracellular			NULL	LME6 cells	0	NULL	NULL	NULL	gw60_jbiolchem_276_29_27129_s_5	11369765	Treatment with exogenous C2-ceramide and sphingosine led to cell death in both LM and LME6, and treatment of the LME6 cells with MNNG resulted in a transient increase in intracellular ceramide of ~50% over a period of 3 h.	transcription
67764	1	336124	7	NULL	NULL	NULL	NULL	C2-ceramide 	Chemical	exogenous	lead to					cell death	Process				NULL	LM 	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_29_27129_s_5	11369765	Treatment with exogenous C2-ceramide and sphingosine led to cell death in both LM and LME6, and treatment of the LME6 cells with MNNG resulted in a transient increase in intracellular ceramide of ~50% over a period of 3 h.	transcription
67765	2	336124	7	NULL	NULL	0	NULL	C2-ceramide	Chemical	exogenous	lead to					cell death	Process				NULL	LME6 cells	0	NULL	NULL	NULL	gw60_jbiolchem_276_29_27129_s_5	11369765	Treatment with exogenous C2-ceramide and sphingosine led to cell death in both LM and LME6, and treatment of the LME6 cells with MNNG resulted in a transient increase in intracellular ceramide of ~50% over a period of 3 h.	transcription
67766	3	336124	7	NULL	NULL	NULL	NULL	sphingosine	Chemical	exogenous	lead to					cell death	Process				NULL	LM	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_29_27129_s_5	11369765	Treatment with exogenous C2-ceramide and sphingosine led to cell death in both LM and LME6, and treatment of the LME6 cells with MNNG resulted in a transient increase in intracellular ceramide of ~50% over a period of 3 h.	transcription
67767	4	336124	7	NULL	NULL	0	NULL	sphingosine	Chemical	exogenous	lead to					cell death	Process				NULL	LME6 cells	0	NULL	NULL	NULL	gw60_jbiolchem_276_29_27129_s_5	11369765	Treatment with exogenous C2-ceramide and sphingosine led to cell death in both LM and LME6, and treatment of the LME6 cells with MNNG resulted in a transient increase in intracellular ceramide of ~50% over a period of 3 h.	transcription
67768	5	336124	7	NULL	NULL	NULL	NULL	MNNG	Chemical		increase					ceramide	Chemical	intracellular			NULL	LME6 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_276_29_27129_s_5	11369765	Treatment with exogenous C2-ceramide and sphingosine led to cell death in both LM and LME6, and treatment of the LME6 cells with MNNG resulted in a transient increase in intracellular ceramide of ~50% over a period of 3 h.	transcription
66785	1	336125	5	NULL	NULL	NULL	NULL	UV irradiation			activates		dose dependently			AP-1	GP	transactivation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_44_27753_s_50	9346918	The results showed that, in addition to UV irradiation, both SMase and C2-ceramide induced the transactivation of AP-1 activity in a dose-dependent manner (Fig.  1), whereas sphingosine, a metabolite of ceramide, did not induce AP-1 activity (Fig.  1).	transcription
66786	2	336125	5	NULL	NULL	NULL	NULL	SMase	GP		activates		dose dependently			AP-1	GP	transactivation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_44_27753_s_50	9346918	The results showed that, in addition to UV irradiation, both SMase and C2-ceramide induced the transactivation of AP-1 activity in a dose-dependent manner (Fig.  1), whereas sphingosine, a metabolite of ceramide, did not induce AP-1 activity (Fig.  1).	transcription
66787	3	336125	5	NULL	NULL	0	NULL	C2-ceramide	Chemical		activates		dose dependently			AP-1	GP	transactivation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27753_s_50	9346918	The results showed that, in addition to UV irradiation, both SMase and C2-ceramide induced the transactivation of AP-1 activity in a dose-dependent manner (Fig.  1), whereas sphingosine, a metabolite of ceramide, did not induce AP-1 activity (Fig.  1).	transcription
66788	4	336125	5	NULL	NULL	0	NULL	sphingosine	Chemical		is a metabolite of					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27753_s_50	9346918	The results showed that, in addition to UV irradiation, both SMase and C2-ceramide induced the transactivation of AP-1 activity in a dose-dependent manner (Fig.  1), whereas sphingosine, a metabolite of ceramide, did not induce AP-1 activity (Fig.  1).	transcription
66789	5	336125	5	NULL	NULL	0	NULL	sphingosine	Chemical		does not activate					AP-1	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27753_s_50	9346918	The results showed that, in addition to UV irradiation, both SMase and C2-ceramide induced the transactivation of AP-1 activity in a dose-dependent manner (Fig.  1), whereas sphingosine, a metabolite of ceramide, did not induce AP-1 activity (Fig.  1).	transcription
67769	1	336125	7	NULL	NULL	0	NULL	SMase	GP		induce		dose-dependently			AP-1 activity 	Process	transactivation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27753_s_50	9346918	The results showed that, in addition to UV irradiation, both SMase and C2-ceramide induced the transactivation of AP-1 activity in a dose-dependent manner (Fig.  1), whereas sphingosine, a metabolite of ceramide, did not induce AP-1 activity (Fig.  1).	transcription
67770	2	336125	7	NULL	NULL	NULL	NULL	C2-ceramide	Chemical		induce		dose-dependently			AP-1 activity 	Process	transactivation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_44_27753_s_50	9346918	The results showed that, in addition to UV irradiation, both SMase and C2-ceramide induced the transactivation of AP-1 activity in a dose-dependent manner (Fig.  1), whereas sphingosine, a metabolite of ceramide, did not induce AP-1 activity (Fig.  1).	transcription
67771	3	336125	7	NULL	NULL	0	NULL	sphingosine	Chemical		is a metabolite of					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27753_s_50	9346918	The results showed that, in addition to UV irradiation, both SMase and C2-ceramide induced the transactivation of AP-1 activity in a dose-dependent manner (Fig.  1), whereas sphingosine, a metabolite of ceramide, did not induce AP-1 activity (Fig.  1).	transcription
67772	4	336125	7	NULL	NULL	0	NULL	sphingosine	Chemical		does not induce					AP-1 activity 	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27753_s_50	9346918	The results showed that, in addition to UV irradiation, both SMase and C2-ceramide induced the transactivation of AP-1 activity in a dose-dependent manner (Fig.  1), whereas sphingosine, a metabolite of ceramide, did not induce AP-1 activity (Fig.  1).	transcription
66790	1	336126	5	NULL	NULL	0	NULL	ceramide	Chemical		is converted to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_8_4836_s_133	9030540	Next, to determine whether blocking the conversion of ceramide to sphingosine would abrogate the negative inotropic effects of TNF-alpha, the cells were pretreated (60 min) with a specific inhibitor of ceramidase:  n-oleoylethanolamine (NOE) ( 28).	transcription
66791	2	336126	5	NULL	NULL	0	NULL	statement 1	Process	blocking of	abrogates		possibly			TNF-alpha	GP	negative inotropic effects of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_8_4836_s_133	9030540	Next, to determine whether blocking the conversion of ceramide to sphingosine would abrogate the negative inotropic effects of TNF-alpha, the cells were pretreated (60 min) with a specific inhibitor of ceramidase:  n-oleoylethanolamine (NOE) ( 28).	transcription
66792	3	336126	5	NULL	NULL	NULL	NULL	NOE	Chemical		is					n-oleoylethanolamine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_8_4836_s_133	9030540	Next, to determine whether blocking the conversion of ceramide to sphingosine would abrogate the negative inotropic effects of TNF-alpha, the cells were pretreated (60 min) with a specific inhibitor of ceramidase:  n-oleoylethanolamine (NOE) ( 28).	transcription
66793	4	336126	5	NULL	NULL	0	NULL	NOE	Chemical		is an inhibitor of					ceramidase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_8_4836_s_133	9030540	Next, to determine whether blocking the conversion of ceramide to sphingosine would abrogate the negative inotropic effects of TNF-alpha, the cells were pretreated (60 min) with a specific inhibitor of ceramidase:  n-oleoylethanolamine (NOE) ( 28).	transcription
67773	1	336126	7	NULL	NULL	0	NULL	NOE	Chemical		is an inhibitor of					ceramidase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_8_4836_s_133	9030540	Next, to determine whether blocking the conversion of ceramide to sphingosine would abrogate the negative inotropic effects of TNF-alpha, the cells were pretreated (60 min) with a specific inhibitor of ceramidase:  n-oleoylethanolamine (NOE) ( 28).	transcription
67774	2	336126	7	NULL	NULL	0	NULL	NOE	Chemical		is dependent on					n-oleoylethanolamine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_8_4836_s_133	9030540	Next, to determine whether blocking the conversion of ceramide to sphingosine would abrogate the negative inotropic effects of TNF-alpha, the cells were pretreated (60 min) with a specific inhibitor of ceramidase:  n-oleoylethanolamine (NOE) ( 28).	transcription
66794	1	336127	5	NULL	NULL	0	NULL	PAP2	GP	rat;;liver	is inhibited by					lyso-PA	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10361_s_9	9099673	Like rat liver PAP2, the Mg2+-independent PA phosphatase activity of DGPP phosphatase purified from  S. cerevisiae was inhibited by lyso-PA, sphingosine 1-phosphate, and ceramide 1-phosphate.	transcription
66795	2	336127	5	NULL	NULL	0	NULL	PAP2	GP	rat;;liver	is inhibited by					sphingosine 1-phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10361_s_9	9099673	Like rat liver PAP2, the Mg2+-independent PA phosphatase activity of DGPP phosphatase purified from  S. cerevisiae was inhibited by lyso-PA, sphingosine 1-phosphate, and ceramide 1-phosphate.	transcription
66796	3	336127	5	NULL	NULL	0	NULL	PAP2	GP	rat;;liver	is inhibited by					ceramide-1-phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10361_s_9	9099673	Like rat liver PAP2, the Mg2+-independent PA phosphatase activity of DGPP phosphatase purified from  S. cerevisiae was inhibited by lyso-PA, sphingosine 1-phosphate, and ceramide 1-phosphate.	transcription
66797	4	336127	5	NULL	NULL	0	NULL	DGPP phosphatase	GP	S. cerevisiae	activates					PA phosphatase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10361_s_9	9099673	Like rat liver PAP2, the Mg2+-independent PA phosphatase activity of DGPP phosphatase purified from  S. cerevisiae was inhibited by lyso-PA, sphingosine 1-phosphate, and ceramide 1-phosphate.	transcription
66798	5	336127	5	NULL	NULL	0	NULL	statement 4	Process		is independent of					Mg2+	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10361_s_9	9099673	Like rat liver PAP2, the Mg2+-independent PA phosphatase activity of DGPP phosphatase purified from  S. cerevisiae was inhibited by lyso-PA, sphingosine 1-phosphate, and ceramide 1-phosphate.	transcription
66799	6	336127	5	NULL	NULL	0	NULL	statement 4	Process		is inhibited by					lyso-PA	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10361_s_9	9099673	Like rat liver PAP2, the Mg2+-independent PA phosphatase activity of DGPP phosphatase purified from  S. cerevisiae was inhibited by lyso-PA, sphingosine 1-phosphate, and ceramide 1-phosphate.	transcription
66800	7	336127	5	NULL	NULL	0	NULL	statement 4	Process		is inhibited by					sphingosine 1-phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10361_s_9	9099673	Like rat liver PAP2, the Mg2+-independent PA phosphatase activity of DGPP phosphatase purified from  S. cerevisiae was inhibited by lyso-PA, sphingosine 1-phosphate, and ceramide 1-phosphate.	transcription
66801	8	336127	5	NULL	NULL	0	NULL	statement 4	Process		is inhibited by					ceramide-1-phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10361_s_9	9099673	Like rat liver PAP2, the Mg2+-independent PA phosphatase activity of DGPP phosphatase purified from  S. cerevisiae was inhibited by lyso-PA, sphingosine 1-phosphate, and ceramide 1-phosphate.	transcription
67775	1	336127	7	NULL	NULL	NULL	NULL	DGPP phosphatase	GP	Mg2+-independent PA phosphatase activity of;; purified from S. cerevisiae	is independent of					Mg2+	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_16_10361_s_9	9099673	Like rat liver PAP2, the Mg2+-independent PA phosphatase activity of DGPP phosphatase purified from  S. cerevisiae was inhibited by lyso-PA, sphingosine 1-phosphate, and ceramide 1-phosphate.	transcription
67776	2	336127	7	NULL	NULL	0	NULL	lyso-PA	Chemical		inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10361_s_9	9099673	Like rat liver PAP2, the Mg2+-independent PA phosphatase activity of DGPP phosphatase purified from  S. cerevisiae was inhibited by lyso-PA, sphingosine 1-phosphate, and ceramide 1-phosphate.	transcription
67777	3	336127	7	NULL	NULL	0	NULL	sphingosine 1-phosphate	Chemical		inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10361_s_9	9099673	Like rat liver PAP2, the Mg2+-independent PA phosphatase activity of DGPP phosphatase purified from  S. cerevisiae was inhibited by lyso-PA, sphingosine 1-phosphate, and ceramide 1-phosphate.	transcription
67778	4	336127	7	NULL	NULL	0	NULL	ceramide 1-phosphate	Chemical		inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_16_10361_s_9	9099673	Like rat liver PAP2, the Mg2+-independent PA phosphatase activity of DGPP phosphatase purified from  S. cerevisiae was inhibited by lyso-PA, sphingosine 1-phosphate, and ceramide 1-phosphate.	transcription
66802	1	336128	5	NULL	NULL	0	NULL	sphingosine	Chemical	elevation of;;endogenous	is caused by					fumonisin B1	Chemical	addition of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_9_5640_s_8	9038174	Elevation of endogenous sphinganine by a second method (addition of fumonisin B1, an inhibitor of ceramide synthase) also reduced [3]PDBu binding; therefore, elevations in sphingosine and sphinganine can both affect PKC.	transcription
66803	2	336128	5	NULL	NULL	0	NULL	fumonisin B1	Chemical		is an inhibitor of					ceramide synthase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_9_5640_s_8	9038174	Elevation of endogenous sphinganine by a second method (addition of fumonisin B1, an inhibitor of ceramide synthase) also reduced [3]PDBu binding; therefore, elevations in sphingosine and sphinganine can both affect PKC.	transcription
66804	3	336128	5	NULL	NULL	0	NULL	statement 1	Process		reduce					PDBu	Chemical	binding of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_9_5640_s_8	9038174	Elevation of endogenous sphinganine by a second method (addition of fumonisin B1, an inhibitor of ceramide synthase) also reduced [3]PDBu binding; therefore, elevations in sphingosine and sphinganine can both affect PKC.	transcription
66805	4	336128	5	NULL	NULL	0	NULL	sphingosine	Chemical	elevation of	affect					PKC	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_9_5640_s_8	9038174	Elevation of endogenous sphinganine by a second method (addition of fumonisin B1, an inhibitor of ceramide synthase) also reduced [3]PDBu binding; therefore, elevations in sphingosine and sphinganine can both affect PKC.	transcription
66806	5	336128	5	NULL	NULL	0	NULL	sphinganine	Chemical	elevation of	affects					PKC	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_9_5640_s_8	9038174	Elevation of endogenous sphinganine by a second method (addition of fumonisin B1, an inhibitor of ceramide synthase) also reduced [3]PDBu binding; therefore, elevations in sphingosine and sphinganine can both affect PKC.	transcription
67779	1	336128	7	NULL	NULL	0	NULL	fumonisin B1	Chemical		is an inhibitor of					ceramide synthase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_9_5640_s_8	9038174	Elevation of endogenous sphinganine by a second method (addition of fumonisin B1, an inhibitor of ceramide synthase) also reduced [3]PDBu binding; therefore, elevations in sphingosine and sphinganine can both affect PKC.	transcription
67780	2	336128	7	NULL	NULL	NULL	NULL	sphinganine 	Chemical	elevation of endogenous	reduce					PDBu	Chemical	binding of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_9_5640_s_8	9038174	Elevation of endogenous sphinganine by a second method (addition of fumonisin B1, an inhibitor of ceramide synthase) also reduced [3]PDBu binding; therefore, elevations in sphingosine and sphinganine can both affect PKC.	transcription
67781	3	336128	7	NULL	NULL	0	NULL	sphingosine	Chemical	elevation in	affect					PKC	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_9_5640_s_8	9038174	Elevation of endogenous sphinganine by a second method (addition of fumonisin B1, an inhibitor of ceramide synthase) also reduced [3]PDBu binding; therefore, elevations in sphingosine and sphinganine can both affect PKC.	transcription
67782	4	336128	7	NULL	NULL	NULL	NULL	sphinganine	Chemical	elevation in	affect					PKC	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_9_5640_s_8	9038174	Elevation of endogenous sphinganine by a second method (addition of fumonisin B1, an inhibitor of ceramide synthase) also reduced [3]PDBu binding; therefore, elevations in sphingosine and sphinganine can both affect PKC.	transcription
66807	1	336129	5	NULL	NULL	0	NULL	COS-7 cells	Cell		treated with					sphingomyelinase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_52_41201_s_249	10995762	We next wanted to determine whether transfected PDK1 could become activated in COS-7 cells treated for 30 min with 1 unit/ml sphingomyelinase, which catalyzes the breakdown of sphingomyelin to form ceramide and subsequently sphingosine.	transcription
66808	2	336129	5	NULL	NULL	0	NULL	PDK1	GP	transfected	is activated in		possibly			statement 1	Cell				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_52_41201_s_249	10995762	We next wanted to determine whether transfected PDK1 could become activated in COS-7 cells treated for 30 min with 1 unit/ml sphingomyelinase, which catalyzes the breakdown of sphingomyelin to form ceramide and subsequently sphingosine.	transcription
66809	3	336129	5	NULL	NULL	0	NULL	sphingomyelin	Chemical		broken down into					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_52_41201_s_249	10995762	We next wanted to determine whether transfected PDK1 could become activated in COS-7 cells treated for 30 min with 1 unit/ml sphingomyelinase, which catalyzes the breakdown of sphingomyelin to form ceramide and subsequently sphingosine.	transcription
66810	4	336129	5	NULL	NULL	0	NULL	sphingomyelin	Chemical		broken down into					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_52_41201_s_249	10995762	We next wanted to determine whether transfected PDK1 could become activated in COS-7 cells treated for 30 min with 1 unit/ml sphingomyelinase, which catalyzes the breakdown of sphingomyelin to form ceramide and subsequently sphingosine.	transcription
66811	5	336129	5	NULL	NULL	0	NULL	statement 3	Process		subsequent to					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_52_41201_s_249	10995762	We next wanted to determine whether transfected PDK1 could become activated in COS-7 cells treated for 30 min with 1 unit/ml sphingomyelinase, which catalyzes the breakdown of sphingomyelin to form ceramide and subsequently sphingosine.	transcription
66812	6	336129	5	NULL	NULL	NULL	NULL	sphingomyelinase	GP		catalyzes					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_52_41201_s_249	10995762	We next wanted to determine whether transfected PDK1 could become activated in COS-7 cells treated for 30 min with 1 unit/ml sphingomyelinase, which catalyzes the breakdown of sphingomyelin to form ceramide and subsequently sphingosine.	transcription
67783	1	336129	7	NULL	NULL	NULL	NULL	sphingomyelin	Chemical		forms					ceramide	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_52_41201_s_249	10995762	We next wanted to determine whether transfected PDK1 could become activated in COS-7 cells treated for 30 min with 1 unit/ml sphingomyelinase, which catalyzes the breakdown of sphingomyelin to form ceramide and subsequently sphingosine.	transcription
67784	2	336129	7	NULL	NULL	0	NULL	ceramide	Chemical		 forms		subsequently			sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_52_41201_s_249	10995762	We next wanted to determine whether transfected PDK1 could become activated in COS-7 cells treated for 30 min with 1 unit/ml sphingomyelinase, which catalyzes the breakdown of sphingomyelin to form ceramide and subsequently sphingosine.	transcription
67785	3	336129	7	NULL	NULL	0	NULL	sphingomyelinase	GP		catalyze					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_52_41201_s_249	10995762	We next wanted to determine whether transfected PDK1 could become activated in COS-7 cells treated for 30 min with 1 unit/ml sphingomyelinase, which catalyzes the breakdown of sphingomyelin to form ceramide and subsequently sphingosine.	transcription
67786	4	336129	7	NULL	NULL	0	NULL	sphingomyelinase	GP		catalyze					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_52_41201_s_249	10995762	We next wanted to determine whether transfected PDK1 could become activated in COS-7 cells treated for 30 min with 1 unit/ml sphingomyelinase, which catalyzes the breakdown of sphingomyelin to form ceramide and subsequently sphingosine.	transcription
66813	1	336130	5	NULL	NULL	0	NULL	ceramide	Chemical		is hydrolyzed to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_70	10747891	Sphingosine, the product of ceramide hydrolysis catalyzed by ceramidases, has been shown to be rapidly produced during TNFalpha-mediated apoptosis in human neutrophils ( 28) and rat cardiomyocytes ( 32).	transcription
66814	2	336130	5	NULL	NULL	0	NULL	ceramidases	GP		catalyzes					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_70	10747891	Sphingosine, the product of ceramide hydrolysis catalyzed by ceramidases, has been shown to be rapidly produced during TNFalpha-mediated apoptosis in human neutrophils ( 28) and rat cardiomyocytes ( 32).	transcription
66815	3	336130	5	NULL	NULL	0	NULL	apoptosis	Process		is mediated by					TNFalpha	GP				NULL	human neutrophils	0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_70	10747891	Sphingosine, the product of ceramide hydrolysis catalyzed by ceramidases, has been shown to be rapidly produced during TNFalpha-mediated apoptosis in human neutrophils ( 28) and rat cardiomyocytes ( 32).	transcription
66816	4	336130	5	NULL	NULL	0	NULL	apoptosis	Process		is mediated by					TNFalpha	GP				NULL	rat cardiomyocytes	0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_70	10747891	Sphingosine, the product of ceramide hydrolysis catalyzed by ceramidases, has been shown to be rapidly produced during TNFalpha-mediated apoptosis in human neutrophils ( 28) and rat cardiomyocytes ( 32).	transcription
66817	5	336130	5	NULL	NULL	0	NULL	statement 3	Process		produce		rapidly			sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_70	10747891	Sphingosine, the product of ceramide hydrolysis catalyzed by ceramidases, has been shown to be rapidly produced during TNFalpha-mediated apoptosis in human neutrophils ( 28) and rat cardiomyocytes ( 32).	transcription
66818	6	336130	5	NULL	NULL	0	NULL	statement 4	Process		produce		rapidly			sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_70	10747891	Sphingosine, the product of ceramide hydrolysis catalyzed by ceramidases, has been shown to be rapidly produced during TNFalpha-mediated apoptosis in human neutrophils ( 28) and rat cardiomyocytes ( 32).	transcription
67787	1	336130	7	NULL	NULL	0	NULL	ceramide	Chemical	hydrolysis of	produce					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_70	10747891	Sphingosine, the product of ceramide hydrolysis catalyzed by ceramidases, has been shown to be rapidly produced during TNFalpha-mediated apoptosis in human neutrophils ( 28) and rat cardiomyocytes ( 32).	transcription
67788	2	336130	7	NULL	NULL	0	NULL	ceramidases	GP		catalyze					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_70	10747891	Sphingosine, the product of ceramide hydrolysis catalyzed by ceramidases, has been shown to be rapidly produced during TNFalpha-mediated apoptosis in human neutrophils ( 28) and rat cardiomyocytes ( 32).	transcription
67789	3	336130	7	NULL	NULL	NULL	NULL	TNFalpha	GP		mediate					apoptosis	Process				NULL	human neutrophils	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_70	10747891	Sphingosine, the product of ceramide hydrolysis catalyzed by ceramidases, has been shown to be rapidly produced during TNFalpha-mediated apoptosis in human neutrophils ( 28) and rat cardiomyocytes ( 32).	transcription
67790	4	336130	7	NULL	NULL	0	NULL	TNFalpha	GP		mediate					apoptosis	Process				NULL	rat cardiomyocytes	0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_70	10747891	Sphingosine, the product of ceramide hydrolysis catalyzed by ceramidases, has been shown to be rapidly produced during TNFalpha-mediated apoptosis in human neutrophils ( 28) and rat cardiomyocytes ( 32).	transcription
67791	5	336130	7	NULL	NULL	0	NULL	statement 1	Process		occur during		rapidly			statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_70	10747891	Sphingosine, the product of ceramide hydrolysis catalyzed by ceramidases, has been shown to be rapidly produced during TNFalpha-mediated apoptosis in human neutrophils ( 28) and rat cardiomyocytes ( 32).	transcription
67792	6	336130	7	NULL	NULL	0	NULL	statement 1	Process		occur during		rapidly			statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_70	10747891	Sphingosine, the product of ceramide hydrolysis catalyzed by ceramidases, has been shown to be rapidly produced during TNFalpha-mediated apoptosis in human neutrophils ( 28) and rat cardiomyocytes ( 32).	transcription
66819	1	336131	5	NULL	NULL	0	NULL	Bcl-2	GP	overexpression of	protects against					apoptotic stimuli		diverse			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_106	10747891	Because overexpression of Bcl-2 or Bcl-xL protects against diverse apoptotic stimuli, including ceramide-induced apoptosis ( 41-46), it was important to determine whether the effects of sphingosine were also blocked by these proteins.	transcription
66820	2	336131	5	NULL	NULL	0	NULL	Bcl-xL	GP	overexpression of	protects against					apoptotic stimuli		diverse			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_106	10747891	Because overexpression of Bcl-2 or Bcl-xL protects against diverse apoptotic stimuli, including ceramide-induced apoptosis ( 41-46), it was important to determine whether the effects of sphingosine were also blocked by these proteins.	transcription
66821	3	336131	5	NULL	NULL	NULL	NULL	apoptosis	Process		is induced by					ceramide	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_106	10747891	Because overexpression of Bcl-2 or Bcl-xL protects against diverse apoptotic stimuli, including ceramide-induced apoptosis ( 41-46), it was important to determine whether the effects of sphingosine were also blocked by these proteins.	transcription
66822	4	336131	5	NULL	NULL	0	NULL	statement 1	Process		includes					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_106	10747891	Because overexpression of Bcl-2 or Bcl-xL protects against diverse apoptotic stimuli, including ceramide-induced apoptosis ( 41-46), it was important to determine whether the effects of sphingosine were also blocked by these proteins.	transcription
66823	5	336131	5	NULL	NULL	0	NULL	statement 2	Process		includes					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_106	10747891	Because overexpression of Bcl-2 or Bcl-xL protects against diverse apoptotic stimuli, including ceramide-induced apoptosis ( 41-46), it was important to determine whether the effects of sphingosine were also blocked by these proteins.	transcription
66824	6	336131	5	NULL	NULL	0	NULL	Bcl-xL	GP		blocks		possibly			sphingosine	Chemical	effects of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_106	10747891	Because overexpression of Bcl-2 or Bcl-xL protects against diverse apoptotic stimuli, including ceramide-induced apoptosis ( 41-46), it was important to determine whether the effects of sphingosine were also blocked by these proteins.	transcription
66825	7	336131	5	NULL	NULL	NULL	NULL	Bcl-2	GP		blocks		possibly			sphingosine	Chemical	effects of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_106	10747891	Because overexpression of Bcl-2 or Bcl-xL protects against diverse apoptotic stimuli, including ceramide-induced apoptosis ( 41-46), it was important to determine whether the effects of sphingosine were also blocked by these proteins.	transcription
67808	1	336131	7	NULL	NULL	0	NULL	ceramide	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_106	10747891	Because overexpression of Bcl-2 or Bcl-xL protects against diverse apoptotic stimuli, including ceramide-induced apoptosis ( 41-46), it was important to determine whether the effects of sphingosine were also blocked by these proteins.	transcription
67809	2	336131	7	NULL	NULL	0	NULL	Bcl-2	GP	overexpression of	protects					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_106	10747891	Because overexpression of Bcl-2 or Bcl-xL protects against diverse apoptotic stimuli, including ceramide-induced apoptosis ( 41-46), it was important to determine whether the effects of sphingosine were also blocked by these proteins.	transcription
67810	3	336131	7	NULL	NULL	0	NULL	Bcl-xL	GP	overexpression of	protects					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_106	10747891	Because overexpression of Bcl-2 or Bcl-xL protects against diverse apoptotic stimuli, including ceramide-induced apoptosis ( 41-46), it was important to determine whether the effects of sphingosine were also blocked by these proteins.	transcription
67811	4	336131	7	NULL	NULL	0	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_106	10747891	Because overexpression of Bcl-2 or Bcl-xL protects against diverse apoptotic stimuli, including ceramide-induced apoptosis ( 41-46), it was important to determine whether the effects of sphingosine were also blocked by these proteins.	transcription
66826	1	336132	5	NULL	NULL	0	NULL	caspase	GP	activation of	is required for		potentially			ceramide	Chemical	early generation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_132	10747891	To assess whether caspase activation was required for early ceramide and sphingosine generation triggered by anti-Fas mAb, we utilized the pharmacological peptide ZVAD-fmk, a competitive inhibitor of all caspases ( 50).	transcription
66827	2	336132	5	NULL	NULL	0	NULL	caspase	GP	activation of	is required for		potentially			sphingosine	Chemical	early generation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_132	10747891	To assess whether caspase activation was required for early ceramide and sphingosine generation triggered by anti-Fas mAb, we utilized the pharmacological peptide ZVAD-fmk, a competitive inhibitor of all caspases ( 50).	transcription
66828	3	336132	5	NULL	NULL	NULL	NULL	ZVAD-fmk 	AminoAcid		is an inhibitor of		competitive			caspases	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_132	10747891	To assess whether caspase activation was required for early ceramide and sphingosine generation triggered by anti-Fas mAb, we utilized the pharmacological peptide ZVAD-fmk, a competitive inhibitor of all caspases ( 50).	transcription
66829	4	336132	5	NULL	NULL	0	NULL	ZVAD-fmk	AminoAcid		is a type of					pharmacological peptide 	AminoAcid				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_132	10747891	To assess whether caspase activation was required for early ceramide and sphingosine generation triggered by anti-Fas mAb, we utilized the pharmacological peptide ZVAD-fmk, a competitive inhibitor of all caspases ( 50).	transcription
67812	1	336132	7	NULL	NULL	0	NULL	anti-Fas mAb	GP		trigger					ceramide	Chemical	generation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_132	10747891	To assess whether caspase activation was required for early ceramide and sphingosine generation triggered by anti-Fas mAb, we utilized the pharmacological peptide ZVAD-fmk, a competitive inhibitor of all caspases ( 50).	transcription
67813	2	336132	7	NULL	NULL	0	NULL	anti-Fas mAb	GP		trigger					sphingosine	Chemical	generation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_132	10747891	To assess whether caspase activation was required for early ceramide and sphingosine generation triggered by anti-Fas mAb, we utilized the pharmacological peptide ZVAD-fmk, a competitive inhibitor of all caspases ( 50).	transcription
67814	3	336132	7	NULL	NULL	NULL	NULL	ZVAD-fmk	AminoAcid		 inhibitor of		competitive			caspases	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_132	10747891	To assess whether caspase activation was required for early ceramide and sphingosine generation triggered by anti-Fas mAb, we utilized the pharmacological peptide ZVAD-fmk, a competitive inhibitor of all caspases ( 50).	transcription
67815	4	336132	7	NULL	NULL	0	NULL	ZVAD-fmk	AminoAcid		is a type of					pharmacological peptide 	AminoAcid				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_132	10747891	To assess whether caspase activation was required for early ceramide and sphingosine generation triggered by anti-Fas mAb, we utilized the pharmacological peptide ZVAD-fmk, a competitive inhibitor of all caspases ( 50).	transcription
66830	1	336133	5	NULL	NULL	0	NULL	Jurkat cells	Cell		prerteated with					ZVAD-fmk	AminoAcid				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_133	10747891	Pretreatment of Jurkat cells with ZVAD-fmk (25 muM) inhibited early accumulation of ceramide (Fig.  6 B), similar to a previous report ( 20), and sphingosine (Fig.  6 B) induced by anti-Fas mAb.	transcription
66831	2	336133	5	NULL	NULL	0	NULL	statement 1	Process		inhibits					ceramide	Chemical	early accumulation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_133	10747891	Pretreatment of Jurkat cells with ZVAD-fmk (25 muM) inhibited early accumulation of ceramide (Fig.  6 B), similar to a previous report ( 20), and sphingosine (Fig.  6 B) induced by anti-Fas mAb.	transcription
66832	3	336133	5	NULL	NULL	0	NULL	statement 1	Process		inhibits					sphingosine	Chemical	early accumulation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_133	10747891	Pretreatment of Jurkat cells with ZVAD-fmk (25 muM) inhibited early accumulation of ceramide (Fig.  6 B), similar to a previous report ( 20), and sphingosine (Fig.  6 B) induced by anti-Fas mAb.	transcription
66833	4	336133	5	NULL	NULL	0	NULL	sphingosine	Chemical		is induced by					anti-Fas mAb	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_133	10747891	Pretreatment of Jurkat cells with ZVAD-fmk (25 muM) inhibited early accumulation of ceramide (Fig.  6 B), similar to a previous report ( 20), and sphingosine (Fig.  6 B) induced by anti-Fas mAb.	transcription
67816	1	336133	7	NULL	NULL	NULL	NULL	anti-Fas mAb	GP		induce					ceramide	Chemical	early accumulation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_133	10747891	Pretreatment of Jurkat cells with ZVAD-fmk (25 muM) inhibited early accumulation of ceramide (Fig.  6 B), similar to a previous report ( 20), and sphingosine (Fig.  6 B) induced by anti-Fas mAb.	transcription
67817	2	336133	7	NULL	NULL	NULL	NULL	anti-Fas mAb	GP		induce					sphingosine	Chemical	early accumulation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_133	10747891	Pretreatment of Jurkat cells with ZVAD-fmk (25 muM) inhibited early accumulation of ceramide (Fig.  6 B), similar to a previous report ( 20), and sphingosine (Fig.  6 B) induced by anti-Fas mAb.	transcription
67818	3	336133	7	NULL	NULL	0	NULL	ZVAD-fmk	AminoAcid		inhibit					statement 1	Process				NULL	Jurkat cells	0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_133	10747891	Pretreatment of Jurkat cells with ZVAD-fmk (25 muM) inhibited early accumulation of ceramide (Fig.  6 B), similar to a previous report ( 20), and sphingosine (Fig.  6 B) induced by anti-Fas mAb.	transcription
67819	4	336133	7	NULL	NULL	0	NULL	ZVAD-fmk	AminoAcid		inhibit					statement 2	Process				NULL	Jurkat cells	0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_133	10747891	Pretreatment of Jurkat cells with ZVAD-fmk (25 muM) inhibited early accumulation of ceramide (Fig.  6 B), similar to a previous report ( 20), and sphingosine (Fig.  6 B) induced by anti-Fas mAb.	transcription
66834	1	336134	5	NULL	NULL	0	NULL	executioner caspases	GP	activation of	is induced by					ceramide	Chemical	elevation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_167	10747891	Because Bcl-xL overexpression totally blocks activation of executioner caspases induced by ceramide and sphingosine elevations, it was of interest to determine whether these sphingolipid metabolites could also induce cyt  c release.	transcription
66835	2	336134	5	NULL	NULL	0	NULL	executioner caspases	GP	activation of	is induced by					sphingosine	Chemical	elevation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_167	10747891	Because Bcl-xL overexpression totally blocks activation of executioner caspases induced by ceramide and sphingosine elevations, it was of interest to determine whether these sphingolipid metabolites could also induce cyt  c release.	transcription
66836	3	336134	5	NULL	NULL	NULL	NULL	Bcl-xL	GP	overexpression of	blocks		totally			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_167	10747891	Because Bcl-xL overexpression totally blocks activation of executioner caspases induced by ceramide and sphingosine elevations, it was of interest to determine whether these sphingolipid metabolites could also induce cyt  c release.	transcription
66837	4	336134	5	NULL	NULL	0	NULL	Bcl-xL	GP	overexpression of	blocks		totally			statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_167	10747891	Because Bcl-xL overexpression totally blocks activation of executioner caspases induced by ceramide and sphingosine elevations, it was of interest to determine whether these sphingolipid metabolites could also induce cyt  c release.	transcription
66838	5	336134	5	NULL	NULL	0	NULL	ceramide	Chemical		induce		potentially			cyt c	GP	release of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_167	10747891	Because Bcl-xL overexpression totally blocks activation of executioner caspases induced by ceramide and sphingosine elevations, it was of interest to determine whether these sphingolipid metabolites could also induce cyt  c release.	transcription
66839	6	336134	5	NULL	NULL	0	NULL	sphingosine	Chemical		induce		potentially			cyt c	GP	release of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_167	10747891	Because Bcl-xL overexpression totally blocks activation of executioner caspases induced by ceramide and sphingosine elevations, it was of interest to determine whether these sphingolipid metabolites could also induce cyt  c release.	transcription
66840	7	336134	5	NULL	NULL	0	NULL	sphingosine	Chemical		is a type of					sphingolipid metabolite	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_167	10747891	Because Bcl-xL overexpression totally blocks activation of executioner caspases induced by ceramide and sphingosine elevations, it was of interest to determine whether these sphingolipid metabolites could also induce cyt  c release.	transcription
66841	8	336134	5	NULL	NULL	0	NULL	ceramide	Chemical		is a type of					sphingolipid metabolite	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_167	10747891	Because Bcl-xL overexpression totally blocks activation of executioner caspases induced by ceramide and sphingosine elevations, it was of interest to determine whether these sphingolipid metabolites could also induce cyt  c release.	transcription
67820	1	336134	7	NULL	NULL	NULL	NULL	ceramide	Chemical	elevation of	induce					executioner caspases	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_167	10747891	Because Bcl-xL overexpression totally blocks activation of executioner caspases induced by ceramide and sphingosine elevations, it was of interest to determine whether these sphingolipid metabolites could also induce cyt  c release.	transcription
67821	2	336134	7	NULL	NULL	NULL	NULL	sphingosine	Chemical	elevation of	induce					executioner caspases	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_167	10747891	Because Bcl-xL overexpression totally blocks activation of executioner caspases induced by ceramide and sphingosine elevations, it was of interest to determine whether these sphingolipid metabolites could also induce cyt  c release.	transcription
67822	3	336134	7	NULL	NULL	0	NULL	Bcl-xL 	GP	overexpression of	blocks					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_167	10747891	Because Bcl-xL overexpression totally blocks activation of executioner caspases induced by ceramide and sphingosine elevations, it was of interest to determine whether these sphingolipid metabolites could also induce cyt  c release.	transcription
67823	4	336134	7	NULL	NULL	0	NULL	Bcl-xL 	GP	overexpression of	blocks					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_167	10747891	Because Bcl-xL overexpression totally blocks activation of executioner caspases induced by ceramide and sphingosine elevations, it was of interest to determine whether these sphingolipid metabolites could also induce cyt  c release.	transcription
66842	1	336135	5	NULL	NULL	0	NULL	apoptosis	Process		is induced by					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_225	10747891	FasL/as Interaction Is Not Required for Apoptosis Induced by Sphingosine-- Up-regulation of Fas ligand (FasL) has been proposed as a mechanism of ceramide-mediated apoptosis induced by gamma-irradiation or doxorubicin ( 69).	transcription
66843	2	336135	5	NULL	NULL	0	NULL	FasL/Fas	GP	interactions of	is not required for					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_225	10747891	FasL/as Interaction Is Not Required for Apoptosis Induced by Sphingosine-- Up-regulation of Fas ligand (FasL) has been proposed as a mechanism of ceramide-mediated apoptosis induced by gamma-irradiation or doxorubicin ( 69).	transcription
66844	3	336135	5	NULL	NULL	0	NULL	FasL	GP		is					Fas ligand	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_225	10747891	FasL/as Interaction Is Not Required for Apoptosis Induced by Sphingosine-- Up-regulation of Fas ligand (FasL) has been proposed as a mechanism of ceramide-mediated apoptosis induced by gamma-irradiation or doxorubicin ( 69).	transcription
66845	4	336135	5	NULL	NULL	0	NULL	apoptosis	Process		is mediated by					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_225	10747891	FasL/as Interaction Is Not Required for Apoptosis Induced by Sphingosine-- Up-regulation of Fas ligand (FasL) has been proposed as a mechanism of ceramide-mediated apoptosis induced by gamma-irradiation or doxorubicin ( 69).	transcription
66846	5	336135	5	NULL	NULL	0	NULL	gamma-irradiation			induce					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_225	10747891	FasL/as Interaction Is Not Required for Apoptosis Induced by Sphingosine-- Up-regulation of Fas ligand (FasL) has been proposed as a mechanism of ceramide-mediated apoptosis induced by gamma-irradiation or doxorubicin ( 69).	transcription
66847	6	336135	5	NULL	NULL	0	NULL	doxorubicin	Chemical		induce					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_225	10747891	FasL/as Interaction Is Not Required for Apoptosis Induced by Sphingosine-- Up-regulation of Fas ligand (FasL) has been proposed as a mechanism of ceramide-mediated apoptosis induced by gamma-irradiation or doxorubicin ( 69).	transcription
66848	7	336135	5	NULL	NULL	0	NULL	statement 5	Process		is an alternative to					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_225	10747891	FasL/as Interaction Is Not Required for Apoptosis Induced by Sphingosine-- Up-regulation of Fas ligand (FasL) has been proposed as a mechanism of ceramide-mediated apoptosis induced by gamma-irradiation or doxorubicin ( 69).	transcription
66849	8	336135	5	NULL	NULL	0	NULL	FasL	GP	upregulation of	plays a role in					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_225	10747891	FasL/as Interaction Is Not Required for Apoptosis Induced by Sphingosine-- Up-regulation of Fas ligand (FasL) has been proposed as a mechanism of ceramide-mediated apoptosis induced by gamma-irradiation or doxorubicin ( 69).	transcription
67824	1	336135	7	NULL	NULL	0	NULL	sphingosine	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_225	10747891	FasL/as Interaction Is Not Required for Apoptosis Induced by Sphingosine-- Up-regulation of Fas ligand (FasL) has been proposed as a mechanism of ceramide-mediated apoptosis induced by gamma-irradiation or doxorubicin ( 69).	transcription
67825	2	336135	7	NULL	NULL	0	NULL	FasL/as Interaction	Process		is not required for					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_225	10747891	FasL/as Interaction Is Not Required for Apoptosis Induced by Sphingosine-- Up-regulation of Fas ligand (FasL) has been proposed as a mechanism of ceramide-mediated apoptosis induced by gamma-irradiation or doxorubicin ( 69).	transcription
67826	3	336135	7	NULL	NULL	0	NULL	ceramide	Chemical		mediate					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_225	10747891	FasL/as Interaction Is Not Required for Apoptosis Induced by Sphingosine-- Up-regulation of Fas ligand (FasL) has been proposed as a mechanism of ceramide-mediated apoptosis induced by gamma-irradiation or doxorubicin ( 69).	transcription
67827	4	336135	7	NULL	NULL	0	NULL	gamma-irradiation 			induce					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_225	10747891	FasL/as Interaction Is Not Required for Apoptosis Induced by Sphingosine-- Up-regulation of Fas ligand (FasL) has been proposed as a mechanism of ceramide-mediated apoptosis induced by gamma-irradiation or doxorubicin ( 69).	transcription
67828	5	336135	7	NULL	NULL	0	NULL	 doxorubicin	Chemical		induce					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_225	10747891	FasL/as Interaction Is Not Required for Apoptosis Induced by Sphingosine-- Up-regulation of Fas ligand (FasL) has been proposed as a mechanism of ceramide-mediated apoptosis induced by gamma-irradiation or doxorubicin ( 69).	transcription
66873	1	336136	5	NULL	NULL	NULL	NULL	caspase-8	GP		is activated					mitochondria	CellComponent	upstream of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_278	10747891	Hence, we infer that caspase-8 can be activated both upstream and downstream of mitochondria in Fas-induced apoptosis but only downstream of mitochondria in ceramide-and sphingosine-mediated cell death.	transcription
66875	2	336136	5	NULL	NULL	0	NULL	apoptosis	Process		is induced by					Fas					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_278	10747891	Hence, we infer that caspase-8 can be activated both upstream and downstream of mitochondria in Fas-induced apoptosis but only downstream of mitochondria in ceramide-and sphingosine-mediated cell death.	transcription
66876	3	336136	5	NULL	NULL	0	NULL	statement 1	Process		occurs in					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_278	10747891	Hence, we infer that caspase-8 can be activated both upstream and downstream of mitochondria in Fas-induced apoptosis but only downstream of mitochondria in ceramide-and sphingosine-mediated cell death.	transcription
66877	4	336136	5	NULL	NULL	0	NULL	caspase-8	GP		is activated					mitochondria	CellComponent	downstream of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_278	10747891	Hence, we infer that caspase-8 can be activated both upstream and downstream of mitochondria in Fas-induced apoptosis but only downstream of mitochondria in ceramide-and sphingosine-mediated cell death.	transcription
66878	5	336136	5	NULL	NULL	0	NULL	statement 1	Process		occurs in					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_278	10747891	Hence, we infer that caspase-8 can be activated both upstream and downstream of mitochondria in Fas-induced apoptosis but only downstream of mitochondria in ceramide-and sphingosine-mediated cell death.	transcription
66879	6	336136	5	NULL	NULL	0	NULL	cell death	Process		is mediated by					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_278	10747891	Hence, we infer that caspase-8 can be activated both upstream and downstream of mitochondria in Fas-induced apoptosis but only downstream of mitochondria in ceramide-and sphingosine-mediated cell death.	transcription
66880	7	336136	5	NULL	NULL	0	NULL	cell death	Process		is mediated by					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_278	10747891	Hence, we infer that caspase-8 can be activated both upstream and downstream of mitochondria in Fas-induced apoptosis but only downstream of mitochondria in ceramide-and sphingosine-mediated cell death.	transcription
66881	8	336136	5	NULL	NULL	0	NULL	statement 4	Process		occurs in		only			statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_278	10747891	Hence, we infer that caspase-8 can be activated both upstream and downstream of mitochondria in Fas-induced apoptosis but only downstream of mitochondria in ceramide-and sphingosine-mediated cell death.	transcription
66883	9	336136	5	NULL	NULL	0	NULL	statement 4	Process		occurs in		only			statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_278	10747891	Hence, we infer that caspase-8 can be activated both upstream and downstream of mitochondria in Fas-induced apoptosis but only downstream of mitochondria in ceramide-and sphingosine-mediated cell death.	transcription
67829	1	336136	7	NULL	NULL	0	NULL	Fas	GP		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_278	10747891	Hence, we infer that caspase-8 can be activated both upstream and downstream of mitochondria in Fas-induced apoptosis but only downstream of mitochondria in ceramide-and sphingosine-mediated cell death.	transcription
67830	2	336136	7	NULL	NULL	0	NULL	caspase-8	GP	upstream of mitochondria	activated by					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_278	10747891	Hence, we infer that caspase-8 can be activated both upstream and downstream of mitochondria in Fas-induced apoptosis but only downstream of mitochondria in ceramide-and sphingosine-mediated cell death.	transcription
67831	3	336136	7	NULL	NULL	0	NULL	caspase-8	GP	downstream of mitochondria	activated by					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_278	10747891	Hence, we infer that caspase-8 can be activated both upstream and downstream of mitochondria in Fas-induced apoptosis but only downstream of mitochondria in ceramide-and sphingosine-mediated cell death.	transcription
67832	4	336136	7	NULL	NULL	0	NULL	ceramide	Chemical		mediate					cell death	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_278	10747891	Hence, we infer that caspase-8 can be activated both upstream and downstream of mitochondria in Fas-induced apoptosis but only downstream of mitochondria in ceramide-and sphingosine-mediated cell death.	transcription
67833	5	336136	7	NULL	NULL	0	NULL	sphingosine	Chemical		mediate					cell death	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_278	10747891	Hence, we infer that caspase-8 can be activated both upstream and downstream of mitochondria in Fas-induced apoptosis but only downstream of mitochondria in ceramide-and sphingosine-mediated cell death.	transcription
67834	6	336136	7	NULL	NULL	0	NULL	caspase-8	GP	downstream of mitochondria	activated by					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_278	10747891	Hence, we infer that caspase-8 can be activated both upstream and downstream of mitochondria in Fas-induced apoptosis but only downstream of mitochondria in ceramide-and sphingosine-mediated cell death.	transcription
67835	7	336136	7	NULL	NULL	0	NULL	caspase-8	GP	downstream of mitochondria	activated by					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_278	10747891	Hence, we infer that caspase-8 can be activated both upstream and downstream of mitochondria in Fas-induced apoptosis but only downstream of mitochondria in ceramide-and sphingosine-mediated cell death.	transcription
66862	1	336137	5	NULL	NULL	0	NULL	fatty acid	Chemical		is condensed to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_5_3462_s_10	10652340	This study also clearly demonstrated that the purified 94-kDa ceramidase catalyzed the condensation of fatty acid to sphingosine to generate ceramide, but did not catalyze acyl-CoA-dependent acyl-transfer reaction.	transcription
66863	2	336137	5	NULL	NULL	0	NULL	sphingosine	Chemical		is converted to					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_5_3462_s_10	10652340	This study also clearly demonstrated that the purified 94-kDa ceramidase catalyzed the condensation of fatty acid to sphingosine to generate ceramide, but did not catalyze acyl-CoA-dependent acyl-transfer reaction.	transcription
66864	3	336137	5	NULL	NULL	0	NULL	94-kDa ceramidase	GP		catalyzes					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_5_3462_s_10	10652340	This study also clearly demonstrated that the purified 94-kDa ceramidase catalyzed the condensation of fatty acid to sphingosine to generate ceramide, but did not catalyze acyl-CoA-dependent acyl-transfer reaction.	transcription
66865	4	336137	5	NULL	NULL	0	NULL	statement 1	Process		followed by					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_5_3462_s_10	10652340	This study also clearly demonstrated that the purified 94-kDa ceramidase catalyzed the condensation of fatty acid to sphingosine to generate ceramide, but did not catalyze acyl-CoA-dependent acyl-transfer reaction.	transcription
66870	5	336137	5	NULL	NULL	0	NULL	acyl-transfer reaction	Process		is dependent on					acyl-CoA	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_5_3462_s_10	10652340	This study also clearly demonstrated that the purified 94-kDa ceramidase catalyzed the condensation of fatty acid to sphingosine to generate ceramide, but did not catalyze acyl-CoA-dependent acyl-transfer reaction.	transcription
66872	6	336137	5	NULL	NULL	0	NULL	94-kDa ceramidase	GP		does not catalyze					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_5_3462_s_10	10652340	This study also clearly demonstrated that the purified 94-kDa ceramidase catalyzed the condensation of fatty acid to sphingosine to generate ceramide, but did not catalyze acyl-CoA-dependent acyl-transfer reaction.	transcription
67836	1	336137	7	NULL	NULL	0	NULL	fatty acid	Chemical		condense to form					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_5_3462_s_10	10652340	This study also clearly demonstrated that the purified 94-kDa ceramidase catalyzed the condensation of fatty acid to sphingosine to generate ceramide, but did not catalyze acyl-CoA-dependent acyl-transfer reaction.	transcription
67837	2	336137	7	NULL	NULL	0	NULL	statement 1	Process		generate					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_5_3462_s_10	10652340	This study also clearly demonstrated that the purified 94-kDa ceramidase catalyzed the condensation of fatty acid to sphingosine to generate ceramide, but did not catalyze acyl-CoA-dependent acyl-transfer reaction.	transcription
67838	3	336137	7	NULL	NULL	NULL	NULL	ceramidase	GP	purified	catalyze					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3462_s_10	10652340	This study also clearly demonstrated that the purified 94-kDa ceramidase catalyzed the condensation of fatty acid to sphingosine to generate ceramide, but did not catalyze acyl-CoA-dependent acyl-transfer reaction.	transcription
67839	4	336137	7	NULL	NULL	NULL	NULL	ceramidase	GP	purified	does not catalyze					acyl-CoA-dependent acyl-transfer reaction	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_5_3462_s_10	10652340	This study also clearly demonstrated that the purified 94-kDa ceramidase catalyzed the condensation of fatty acid to sphingosine to generate ceramide, but did not catalyze acyl-CoA-dependent acyl-transfer reaction.	transcription
66884	1	336138	5	NULL	NULL	0	NULL	DHS	Chemical		is an inhibitor of		potent			sphingosine kinase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_41_32220_s_229	10915783	Therefore, using DHS, a potent inhibitor of sphingosine kinase, we explored whether the selective stimulation of ceramide for the expression of RAR-alpha and RXR-alpha genes in MC3T3-E1 cells was mediated by SPP.	transcription
66889	2	336138	5	NULL	NULL	NULL	NULL	ceramide	Chemical	selective stimulation of	express					RAR-alpha gene	GP				NULL	MC3T3-E1 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_32220_s_229	10915783	Therefore, using DHS, a potent inhibitor of sphingosine kinase, we explored whether the selective stimulation of ceramide for the expression of RAR-alpha and RXR-alpha genes in MC3T3-E1 cells was mediated by SPP.	transcription
66890	3	336138	5	NULL	NULL	NULL	NULL	SPP	Chemical		mediates		possibly			statement 2	Process				NULL	MC3T3-E1 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_32220_s_229	10915783	Therefore, using DHS, a potent inhibitor of sphingosine kinase, we explored whether the selective stimulation of ceramide for the expression of RAR-alpha and RXR-alpha genes in MC3T3-E1 cells was mediated by SPP.	transcription
66891	4	336138	5	NULL	NULL	0	NULL	ceramide	Chemical	selective stimulation of	express					RXR-alpha gene	GP				NULL	MC3T3-E1 cells	0	NULL	NULL	NULL	gw60_jbiolchem_275_41_32220_s_229	10915783	Therefore, using DHS, a potent inhibitor of sphingosine kinase, we explored whether the selective stimulation of ceramide for the expression of RAR-alpha and RXR-alpha genes in MC3T3-E1 cells was mediated by SPP.	transcription
66892	5	336138	5	NULL	NULL	NULL	NULL	SPP	Chemical		mediates		possibly			statement 4	Process				NULL	MC3T3-E1 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_41_32220_s_229	10915783	Therefore, using DHS, a potent inhibitor of sphingosine kinase, we explored whether the selective stimulation of ceramide for the expression of RAR-alpha and RXR-alpha genes in MC3T3-E1 cells was mediated by SPP.	transcription
67840	1	336138	7	NULL	NULL	0	NULL	DHS	Chemical		potent inhibitor of					sphingosine kinase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_41_32220_s_229	10915783	Therefore, using DHS, a potent inhibitor of sphingosine kinase, we explored whether the selective stimulation of ceramide for the expression of RAR-alpha and RXR-alpha genes in MC3T3-E1 cells was mediated by SPP.	transcription
66893	1	336139	5	NULL	NULL	0	NULL	C -ceramide	Chemical		blocks		completely			SPP	Chemical	effects of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_159	7592842	Furthermore,  C -ceramide, which blocks the effect of SPP completely (  Fig. 1and  Fig. 2), had only a marginal effect on the  inhibition of DNA synthesis induced by sphingosine ( Fig. 3).	transcription
66894	2	336139	5	NULL	NULL	0	NULL	DNA	NucleicAcid	synthesis of	is induced by					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_159	7592842	Furthermore,  C -ceramide, which blocks the effect of SPP completely (  Fig. 1and  Fig. 2), had only a marginal effect on the  inhibition of DNA synthesis induced by sphingosine ( Fig. 3).	transcription
66895	3	336139	5	NULL	NULL	0	NULL	C -ceramide	Chemical		effects		marginal			statement 2	Process	inhibition of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_159	7592842	Furthermore,  C -ceramide, which blocks the effect of SPP completely (  Fig. 1and  Fig. 2), had only a marginal effect on the  inhibition of DNA synthesis induced by sphingosine ( Fig. 3).	transcription
67841	1	336139	7	NULL	NULL	0	NULL	 C -ceramide	Chemical		blocks		completely			SPP	Chemical	effect of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_159	7592842	Furthermore,  C -ceramide, which blocks the effect of SPP completely (  Fig. 1and  Fig. 2), had only a marginal effect on the  inhibition of DNA synthesis induced by sphingosine ( Fig. 3).	transcription
67842	2	336139	7	NULL	NULL	0	NULL	sphingosine	Chemical		induce					DNA synthesis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_159	7592842	Furthermore,  C -ceramide, which blocks the effect of SPP completely (  Fig. 1and  Fig. 2), had only a marginal effect on the  inhibition of DNA synthesis induced by sphingosine ( Fig. 3).	transcription
67843	3	336139	7	NULL	NULL	0	NULL	C -ceramide	Chemical		inhibit		marginally			statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_44_26318_s_159	7592842	Furthermore,  C -ceramide, which blocks the effect of SPP completely (  Fig. 1and  Fig. 2), had only a marginal effect on the  inhibition of DNA synthesis induced by sphingosine ( Fig. 3).	transcription
66912	1	336140	5	NULL	NULL	0	NULL	gangliosides	Chemical		incorporates					carbohydrate moiety	Chemical	homogeneous			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_50_30173_s_181	8530426	These molecular ions suggest the presence of  a series of gangliosides incorporating a homogeneous carbohydrate  moiety,  i.e.  a monoacetylated tetrasaccharide of the  composition AcNeuAc-NeuAc-Hex   linked to a heterogeneous  ceramide portion with C19-C24 fatty acids bound to a C18 sphingosine.	transcription
66913	2	336140	5	NULL	NULL	0	NULL	carbohydrate moiety	Chemical		is a type of					tetrasaccharide	Chemical	monoacetylated			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_50_30173_s_181	8530426	These molecular ions suggest the presence of  a series of gangliosides incorporating a homogeneous carbohydrate  moiety,  i.e.  a monoacetylated tetrasaccharide of the  composition AcNeuAc-NeuAc-Hex   linked to a heterogeneous  ceramide portion with C19-C24 fatty acids bound to a C18 sphingosine.	transcription
66914	3	336140	5	NULL	NULL	0	NULL	AcNeuAc-NeuAc-Hex	Chemical		is the composition of					tetrasaccharide	Chemical	monoacetylated			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_50_30173_s_181	8530426	These molecular ions suggest the presence of  a series of gangliosides incorporating a homogeneous carbohydrate  moiety,  i.e.  a monoacetylated tetrasaccharide of the  composition AcNeuAc-NeuAc-Hex   linked to a heterogeneous  ceramide portion with C19-C24 fatty acids bound to a C18 sphingosine.	transcription
66915	4	336140	5	NULL	NULL	0	NULL	tetrasaccharide	Chemical	monoacetylated	is linked to					ceramide portion	Chemical	heterogeneous			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_50_30173_s_181	8530426	These molecular ions suggest the presence of  a series of gangliosides incorporating a homogeneous carbohydrate  moiety,  i.e.  a monoacetylated tetrasaccharide of the  composition AcNeuAc-NeuAc-Hex   linked to a heterogeneous  ceramide portion with C19-C24 fatty acids bound to a C18 sphingosine.	transcription
66916	5	336140	5	NULL	NULL	0	NULL	C19-C24 fatty acids	Chemical		bind					C18 sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_50_30173_s_181	8530426	These molecular ions suggest the presence of  a series of gangliosides incorporating a homogeneous carbohydrate  moiety,  i.e.  a monoacetylated tetrasaccharide of the  composition AcNeuAc-NeuAc-Hex   linked to a heterogeneous  ceramide portion with C19-C24 fatty acids bound to a C18 sphingosine.	transcription
66917	6	336140	5	NULL	NULL	0	NULL	statement 4	Process		occurs with					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_50_30173_s_181	8530426	These molecular ions suggest the presence of  a series of gangliosides incorporating a homogeneous carbohydrate  moiety,  i.e.  a monoacetylated tetrasaccharide of the  composition AcNeuAc-NeuAc-Hex   linked to a heterogeneous  ceramide portion with C19-C24 fatty acids bound to a C18 sphingosine.	transcription
67844	1	336140	7	NULL	NULL	NULL	NULL	AcNeuAc-NeuAc-Hex 	Chemical		linked to					ceramide with C19-C24 fatty acids	Chemical	heterogeneous			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_50_30173_s_181	8530426	These molecular ions suggest the presence of  a series of gangliosides incorporating a homogeneous carbohydrate  moiety,  i.e.  a monoacetylated tetrasaccharide of the  composition AcNeuAc-NeuAc-Hex   linked to a heterogeneous  ceramide portion with C19-C24 fatty acids bound to a C18 sphingosine.	transcription
67845	2	336140	7	NULL	NULL	NULL	NULL	statement 1	Chemical		bind					C18 sphingosine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_270_50_30173_s_181	8530426	These molecular ions suggest the presence of  a series of gangliosides incorporating a homogeneous carbohydrate  moiety,  i.e.  a monoacetylated tetrasaccharide of the  composition AcNeuAc-NeuAc-Hex   linked to a heterogeneous  ceramide portion with C19-C24 fatty acids bound to a C18 sphingosine.	transcription
67846	3	336140	7	NULL	NULL	0	NULL	AcNeuAc-NeuAc-Hex	Chemical		is a type of					monoacetylated tetrasaccharide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_270_50_30173_s_181	8530426	These molecular ions suggest the presence of  a series of gangliosides incorporating a homogeneous carbohydrate  moiety,  i.e.  a monoacetylated tetrasaccharide of the  composition AcNeuAc-NeuAc-Hex   linked to a heterogeneous  ceramide portion with C19-C24 fatty acids bound to a C18 sphingosine.	transcription
66918	1	336141	5	NULL	NULL	0	NULL	FB1	Chemical		inhibits					sphingosine N-acyltransferase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_20763_s_128	10409615	FB1 inhibits sphingosine  N-acyltransferase (ceramide synthase) in a concentration-dependent manner and thereby interferes with the biosynthesis of all sphingolipids beyond the sphingoid base, in a variety of cells ( 57).	transcription
66919	2	336141	5	NULL	NULL	0	NULL	sphingosine N-acyltransferase	GP		is					ceramide synthase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_20763_s_128	10409615	FB1 inhibits sphingosine  N-acyltransferase (ceramide synthase) in a concentration-dependent manner and thereby interferes with the biosynthesis of all sphingolipids beyond the sphingoid base, in a variety of cells ( 57).	transcription
66920	3	336141	5	NULL	NULL	0	NULL	statement 1	Process		is dependent on					concentration	QuantityOrMeasure				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_20763_s_128	10409615	FB1 inhibits sphingosine  N-acyltransferase (ceramide synthase) in a concentration-dependent manner and thereby interferes with the biosynthesis of all sphingolipids beyond the sphingoid base, in a variety of cells ( 57).	transcription
66921	4	336141	5	NULL	NULL	0	NULL	statement 1	Process		interfere with					sphingolipids	Chemical	biosynthesis of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_20763_s_128	10409615	FB1 inhibits sphingosine  N-acyltransferase (ceramide synthase) in a concentration-dependent manner and thereby interferes with the biosynthesis of all sphingolipids beyond the sphingoid base, in a variety of cells ( 57).	transcription
67847	1	336141	7	NULL	NULL	NULL	NULL	FB1	Chemical		inhibit					sphingosine N-acyltransferase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_30_20763_s_128	10409615	FB1 inhibits sphingosine  N-acyltransferase (ceramide synthase) in a concentration-dependent manner and thereby interferes with the biosynthesis of all sphingolipids beyond the sphingoid base, in a variety of cells ( 57).	transcription
67848	2	336141	7	NULL	NULL	0	NULL	statement 1	Process		depends on					concentration	QuantityOrMeasure				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_20763_s_128	10409615	FB1 inhibits sphingosine  N-acyltransferase (ceramide synthase) in a concentration-dependent manner and thereby interferes with the biosynthesis of all sphingolipids beyond the sphingoid base, in a variety of cells ( 57).	transcription
67849	3	336141	7	NULL	NULL	NULL	NULL	statement 1	Process		interferes with					sphingolipids	Chemical	biosynthesis of			NULL	variety of cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_30_20763_s_128	10409615	FB1 inhibits sphingosine  N-acyltransferase (ceramide synthase) in a concentration-dependent manner and thereby interferes with the biosynthesis of all sphingolipids beyond the sphingoid base, in a variety of cells ( 57).	transcription
67850	4	336141	7	NULL	NULL	0	NULL	sphingosine N-acyltransferase	GP		is					ceramide synthase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_30_20763_s_128	10409615	FB1 inhibits sphingosine  N-acyltransferase (ceramide synthase) in a concentration-dependent manner and thereby interferes with the biosynthesis of all sphingolipids beyond the sphingoid base, in a variety of cells ( 57).	transcription
66922	1	336142	5	NULL	NULL	0	NULL	apoptosis	Process		is induced by					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_37_23722_s_108	9726979	Interestingly, we previously demonstrated that inhibition of ceramide-induced apoptosis by protein kinase C activation results from stimulation of sphingosine kinase and concomitant increase in cellular SPP levels ( 3).	transcription
66923	2	336142	5	NULL	NULL	0	NULL	protein kinase C	GP	activated	inhibits					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_37_23722_s_108	9726979	Interestingly, we previously demonstrated that inhibition of ceramide-induced apoptosis by protein kinase C activation results from stimulation of sphingosine kinase and concomitant increase in cellular SPP levels ( 3).	transcription
66924	3	336142	5	NULL	NULL	0	NULL	sphingosine kinase	GP	stimulation of	results in					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_37_23722_s_108	9726979	Interestingly, we previously demonstrated that inhibition of ceramide-induced apoptosis by protein kinase C activation results from stimulation of sphingosine kinase and concomitant increase in cellular SPP levels ( 3).	transcription
66925	4	336142	5	NULL	NULL	0	NULL	SPP	Chemical	concomitant increase in;;cellular levels of	results in					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_37_23722_s_108	9726979	Interestingly, we previously demonstrated that inhibition of ceramide-induced apoptosis by protein kinase C activation results from stimulation of sphingosine kinase and concomitant increase in cellular SPP levels ( 3).	transcription
67851	1	336142	7	NULL	NULL	0	NULL	 ceramide	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_37_23722_s_108	9726979	Interestingly, we previously demonstrated that inhibition of ceramide-induced apoptosis by protein kinase C activation results from stimulation of sphingosine kinase and concomitant increase in cellular SPP levels ( 3).	transcription
67852	2	336142	7	NULL	NULL	0	NULL	 protein kinase C	GP	activation of	inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_37_23722_s_108	9726979	Interestingly, we previously demonstrated that inhibition of ceramide-induced apoptosis by protein kinase C activation results from stimulation of sphingosine kinase and concomitant increase in cellular SPP levels ( 3).	transcription
67853	3	336142	7	NULL	NULL	0	NULL	statement 2	Process		result from					sphingosine kinase	Chemical	stimulation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_37_23722_s_108	9726979	Interestingly, we previously demonstrated that inhibition of ceramide-induced apoptosis by protein kinase C activation results from stimulation of sphingosine kinase and concomitant increase in cellular SPP levels ( 3).	transcription
67854	4	336142	7	NULL	NULL	0	NULL	statement 2	Process		result from					SPP	Chemical	concomitant increase in levels of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_37_23722_s_108	9726979	Interestingly, we previously demonstrated that inhibition of ceramide-induced apoptosis by protein kinase C activation results from stimulation of sphingosine kinase and concomitant increase in cellular SPP levels ( 3).	transcription
66926	1	336143	5	NULL	NULL	0	NULL	apoptosis	Process		is induced by					nerve growth factor	GP	withdrawal of			NULL	PC12 cells	0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2931_s_230	9446605	Conversely, MAPK activation prevented apoptosis induced by nerve growth factor withdrawal in PC12 cells ( 66) and was required for the suppression of ceramide-induced apoptosis by sphingosine 1-phosphate in HL-60 cells ( 67).	transcription
66927	2	336143	5	NULL	NULL	NULL	NULL	MAPK	GP	activation of	prevents					statement 1	Process				NULL	PC12 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_5_2931_s_230	9446605	Conversely, MAPK activation prevented apoptosis induced by nerve growth factor withdrawal in PC12 cells ( 66) and was required for the suppression of ceramide-induced apoptosis by sphingosine 1-phosphate in HL-60 cells ( 67).	transcription
66928	3	336143	5	NULL	NULL	NULL	NULL	apoptosis	Process		is induced by					ceramide	Chemical				NULL	HL-60 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_5_2931_s_230	9446605	Conversely, MAPK activation prevented apoptosis induced by nerve growth factor withdrawal in PC12 cells ( 66) and was required for the suppression of ceramide-induced apoptosis by sphingosine 1-phosphate in HL-60 cells ( 67).	transcription
66929	4	336143	5	NULL	NULL	0	NULL	sphingosine 1-phosphate	Chemical		suppress					statement 3	Process				NULL	HL-60 cells	0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2931_s_230	9446605	Conversely, MAPK activation prevented apoptosis induced by nerve growth factor withdrawal in PC12 cells ( 66) and was required for the suppression of ceramide-induced apoptosis by sphingosine 1-phosphate in HL-60 cells ( 67).	transcription
66930	5	336143	5	NULL	NULL	0	NULL	MAPK	GP	activation of	is required for					statement 4	Process				NULL	HL-60 cells	0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2931_s_230	9446605	Conversely, MAPK activation prevented apoptosis induced by nerve growth factor withdrawal in PC12 cells ( 66) and was required for the suppression of ceramide-induced apoptosis by sphingosine 1-phosphate in HL-60 cells ( 67).	transcription
67855	1	336143	7	NULL	NULL	0	NULL	nerve growth factor 	GP	withdrawal of	induce					apoptosis	Process				NULL	 PC12 cells 	0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2931_s_230	9446605	Conversely, MAPK activation prevented apoptosis induced by nerve growth factor withdrawal in PC12 cells ( 66) and was required for the suppression of ceramide-induced apoptosis by sphingosine 1-phosphate in HL-60 cells ( 67).	transcription
67856	2	336143	7	NULL	NULL	0	NULL	MAPK	GP	activation of	prevents					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2931_s_230	9446605	Conversely, MAPK activation prevented apoptosis induced by nerve growth factor withdrawal in PC12 cells ( 66) and was required for the suppression of ceramide-induced apoptosis by sphingosine 1-phosphate in HL-60 cells ( 67).	transcription
67857	3	336143	7	NULL	NULL	0	NULL	ceramide	Chemical		induce					apoptosis	Process				NULL	HL-60 cells	0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2931_s_230	9446605	Conversely, MAPK activation prevented apoptosis induced by nerve growth factor withdrawal in PC12 cells ( 66) and was required for the suppression of ceramide-induced apoptosis by sphingosine 1-phosphate in HL-60 cells ( 67).	transcription
67858	4	336143	7	NULL	NULL	0	NULL	sphingosine 1-phosphate	Chemical		suppress					statement 3	Process				NULL	HL-60 cells	0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2931_s_230	9446605	Conversely, MAPK activation prevented apoptosis induced by nerve growth factor withdrawal in PC12 cells ( 66) and was required for the suppression of ceramide-induced apoptosis by sphingosine 1-phosphate in HL-60 cells ( 67).	transcription
67859	5	336143	7	NULL	NULL	NULL	NULL	MAPK	GP	activation of	is required for					statement 4	Process				NULL	HL-60 cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_5_2931_s_230	9446605	Conversely, MAPK activation prevented apoptosis induced by nerve growth factor withdrawal in PC12 cells ( 66) and was required for the suppression of ceramide-induced apoptosis by sphingosine 1-phosphate in HL-60 cells ( 67).	transcription
66931	1	336144	5	NULL	NULL	NULL	NULL	PARP	GP	activation of;;cleavage of	is induced by					Fas	GP	ligation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_88	9446602	Sphingosine 1-Phosphate and TPA Inhibit Activation of PARP Cleavage Induced by Fas Ligation and Ceramide-- Because Fas ligation leads to proteolytic cleavage of PARP ( 12,  25-27), it was of interest to determine whether SPP and TPA could inhibit this cleavage.	transcription
66932	2	336144	5	NULL	NULL	NULL	NULL	PARP	GP	activation of;;cleavage of	is induced by					ceramide	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_88	9446602	Sphingosine 1-Phosphate and TPA Inhibit Activation of PARP Cleavage Induced by Fas Ligation and Ceramide-- Because Fas ligation leads to proteolytic cleavage of PARP ( 12,  25-27), it was of interest to determine whether SPP and TPA could inhibit this cleavage.	transcription
66933	3	336144	5	NULL	NULL	0	NULL	sphingosine 1-phosphate	Chemical		inhibits					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_88	9446602	Sphingosine 1-Phosphate and TPA Inhibit Activation of PARP Cleavage Induced by Fas Ligation and Ceramide-- Because Fas ligation leads to proteolytic cleavage of PARP ( 12,  25-27), it was of interest to determine whether SPP and TPA could inhibit this cleavage.	transcription
66934	4	336144	5	NULL	NULL	0	NULL	sphingosine 1-phosphate	Chemical		inhibits					statement 2	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_88	9446602	Sphingosine 1-Phosphate and TPA Inhibit Activation of PARP Cleavage Induced by Fas Ligation and Ceramide-- Because Fas ligation leads to proteolytic cleavage of PARP ( 12,  25-27), it was of interest to determine whether SPP and TPA could inhibit this cleavage.	transcription
66935	5	336144	5	NULL	NULL	0	NULL	TPA	Chemical		inhibits					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_88	9446602	Sphingosine 1-Phosphate and TPA Inhibit Activation of PARP Cleavage Induced by Fas Ligation and Ceramide-- Because Fas ligation leads to proteolytic cleavage of PARP ( 12,  25-27), it was of interest to determine whether SPP and TPA could inhibit this cleavage.	transcription
66936	6	336144	5	NULL	NULL	0	NULL	TPA	Chemical		inhibits					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_88	9446602	Sphingosine 1-Phosphate and TPA Inhibit Activation of PARP Cleavage Induced by Fas Ligation and Ceramide-- Because Fas ligation leads to proteolytic cleavage of PARP ( 12,  25-27), it was of interest to determine whether SPP and TPA could inhibit this cleavage.	transcription
67860	3	336144	7	NULL	NULL	NULL	NULL	Sphingosine 1-Phosphate	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_88	9446602	Sphingosine 1-Phosphate and TPA Inhibit Activation of PARP Cleavage Induced by Fas Ligation and Ceramide-- Because Fas ligation leads to proteolytic cleavage of PARP ( 12,  25-27), it was of interest to determine whether SPP and TPA could inhibit this cleavage.	transcription
67861	4	336144	7	NULL	NULL	NULL	NULL	TPA	Chemical		inhibit					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_88	9446602	Sphingosine 1-Phosphate and TPA Inhibit Activation of PARP Cleavage Induced by Fas Ligation and Ceramide-- Because Fas ligation leads to proteolytic cleavage of PARP ( 12,  25-27), it was of interest to determine whether SPP and TPA could inhibit this cleavage.	transcription
67862	1	336144	7	NULL	NULL	0	NULL	Fas ligation	Process		induce					PARP	GP	activation of;;cleavage of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_88	9446602	Sphingosine 1-Phosphate and TPA Inhibit Activation of PARP Cleavage Induced by Fas Ligation and Ceramide-- Because Fas ligation leads to proteolytic cleavage of PARP ( 12,  25-27), it was of interest to determine whether SPP and TPA could inhibit this cleavage.	transcription
67863	2	336144	7	NULL	NULL	0	NULL	ceramide	Chemical		induce					PARP	GP	activation of;;cleavage of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_88	9446602	Sphingosine 1-Phosphate and TPA Inhibit Activation of PARP Cleavage Induced by Fas Ligation and Ceramide-- Because Fas ligation leads to proteolytic cleavage of PARP ( 12,  25-27), it was of interest to determine whether SPP and TPA could inhibit this cleavage.	transcription
67864	5	336144	7	NULL	NULL	0	NULL	Sphingosine 1-Phosphate	Chemical		inhibit					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_88	9446602	Sphingosine 1-Phosphate and TPA Inhibit Activation of PARP Cleavage Induced by Fas Ligation and Ceramide-- Because Fas ligation leads to proteolytic cleavage of PARP ( 12,  25-27), it was of interest to determine whether SPP and TPA could inhibit this cleavage.	transcription
67865	6	336144	7	NULL	NULL	0	NULL	TPA	Chemical		inhibit					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_88	9446602	Sphingosine 1-Phosphate and TPA Inhibit Activation of PARP Cleavage Induced by Fas Ligation and Ceramide-- Because Fas ligation leads to proteolytic cleavage of PARP ( 12,  25-27), it was of interest to determine whether SPP and TPA could inhibit this cleavage.	transcription
67866	7	336144	7	NULL	NULL	0	NULL	Fas ligation	Process		leads to					PARP	GP	proteolytic cleavage of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_88	9446602	Sphingosine 1-Phosphate and TPA Inhibit Activation of PARP Cleavage Induced by Fas Ligation and Ceramide-- Because Fas ligation leads to proteolytic cleavage of PARP ( 12,  25-27), it was of interest to determine whether SPP and TPA could inhibit this cleavage.	transcription
66937	1	336145	5	NULL	NULL	0	NULL	programmed cell death	Process		is mediated by					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jclininvest_101_2_301_s_521	9435301	Cuvillier, O., G. Pirianov, B. Kleuser, P.G. Vanek, O.A. Coso, S. Gutkind, and S. Spiegel    (1996) Suppression of ceramide-mediated programmed cell  death by sphingosine-A-phosphate.	transcription
66938	2	336145	5	NULL	NULL	0	NULL	sphingosine-A-phosphate	Chemical		suppress					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jclininvest_101_2_301_s_521	9435301	Cuvillier, O., G. Pirianov, B. Kleuser, P.G. Vanek, O.A. Coso, S. Gutkind, and S. Spiegel    (1996) Suppression of ceramide-mediated programmed cell  death by sphingosine-A-phosphate.	transcription
67867	1	336145	7	NULL	NULL	0	NULL	ceramide	Chemical		mediate					programmed cell death	Process				NULL		0	NULL	NULL	NULL	gw60_jclininvest_101_2_301_s_521	9435301	Cuvillier, O., G. Pirianov, B. Kleuser, P.G. Vanek, O.A. Coso, S. Gutkind, and S. Spiegel    (1996) Suppression of ceramide-mediated programmed cell  death by sphingosine-A-phosphate.	transcription
67868	2	336145	7	NULL	NULL	0	NULL	sphingosine-A-phosphate	Chemical		suppress					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jclininvest_101_2_301_s_521	9435301	Cuvillier, O., G. Pirianov, B. Kleuser, P.G. Vanek, O.A. Coso, S. Gutkind, and S. Spiegel    (1996) Suppression of ceramide-mediated programmed cell  death by sphingosine-A-phosphate.	transcription
66939	1	336146	5	NULL	NULL	0	NULL	ceramide	Chemical		modulate					protein	GP	phosphorylation of			NULL		0	NULL	NULL	NULL	gw60_jlipidres_42_2_301_s_18	11181761	For example, ceramide modulates protein phosphorylation, the activity of protein kinase C (PKC), and phospholipase A2, and mediates signal transduction  ( 2) ( 3), while sphingosine and psychosine are potent inhibitors of PKC  ( 4).	transcription
66940	2	336146	5	NULL	NULL	0	NULL	ceramide	Chemical		modulate					PKC	GP	activity of			NULL		0	NULL	NULL	NULL	gw60_jlipidres_42_2_301_s_18	11181761	For example, ceramide modulates protein phosphorylation, the activity of protein kinase C (PKC), and phospholipase A2, and mediates signal transduction  ( 2) ( 3), while sphingosine and psychosine are potent inhibitors of PKC  ( 4).	transcription
66941	3	336146	5	NULL	NULL	0	NULL	PKC	GP		is					protein kinase C	GP				NULL		0	NULL	NULL	NULL	gw60_jlipidres_42_2_301_s_18	11181761	For example, ceramide modulates protein phosphorylation, the activity of protein kinase C (PKC), and phospholipase A2, and mediates signal transduction  ( 2) ( 3), while sphingosine and psychosine are potent inhibitors of PKC  ( 4).	transcription
66942	4	336146	5	NULL	NULL	0	NULL	ceramide	Chemical		modulate					phospholipase A2	GP				NULL		0	NULL	NULL	NULL	gw60_jlipidres_42_2_301_s_18	11181761	For example, ceramide modulates protein phosphorylation, the activity of protein kinase C (PKC), and phospholipase A2, and mediates signal transduction  ( 2) ( 3), while sphingosine and psychosine are potent inhibitors of PKC  ( 4).	transcription
66943	5	336146	5	NULL	NULL	0	NULL	ceramide	Chemical		mediates					signal transduction	Process				NULL		0	NULL	NULL	NULL	gw60_jlipidres_42_2_301_s_18	11181761	For example, ceramide modulates protein phosphorylation, the activity of protein kinase C (PKC), and phospholipase A2, and mediates signal transduction  ( 2) ( 3), while sphingosine and psychosine are potent inhibitors of PKC  ( 4).	transcription
66944	6	336146	5	NULL	NULL	0	NULL	sphingosine	Chemical		is an inhibitor of		potent			PKC	GP				NULL		0	NULL	NULL	NULL	gw60_jlipidres_42_2_301_s_18	11181761	For example, ceramide modulates protein phosphorylation, the activity of protein kinase C (PKC), and phospholipase A2, and mediates signal transduction  ( 2) ( 3), while sphingosine and psychosine are potent inhibitors of PKC  ( 4).	transcription
66945	7	336146	5	NULL	NULL	0	NULL	psychosine	Chemical		is an inhibitor of		potent			PKC	GP				NULL		0	NULL	NULL	NULL	gw60_jlipidres_42_2_301_s_18	11181761	For example, ceramide modulates protein phosphorylation, the activity of protein kinase C (PKC), and phospholipase A2, and mediates signal transduction  ( 2) ( 3), while sphingosine and psychosine are potent inhibitors of PKC  ( 4).	transcription
67869	1	336146	7	NULL	NULL	0	NULL	ceramide	Chemical		modulates					protein phosphorylation	Process				NULL		0	NULL	NULL	NULL	gw60_jlipidres_42_2_301_s_18	11181761	For example, ceramide modulates protein phosphorylation, the activity of protein kinase C (PKC), and phospholipase A2, and mediates signal transduction  ( 2) ( 3), while sphingosine and psychosine are potent inhibitors of PKC  ( 4).	transcription
67870	2	336146	7	NULL	NULL	0	NULL	ceramide	Chemical		modulates					PKC activity	Process				NULL		0	NULL	NULL	NULL	gw60_jlipidres_42_2_301_s_18	11181761	For example, ceramide modulates protein phosphorylation, the activity of protein kinase C (PKC), and phospholipase A2, and mediates signal transduction  ( 2) ( 3), while sphingosine and psychosine are potent inhibitors of PKC  ( 4).	transcription
67871	3	336146	7	NULL	NULL	0	NULL	ceramide	Chemical		modulates					phospholipase A2	GP				NULL		0	NULL	NULL	NULL	gw60_jlipidres_42_2_301_s_18	11181761	For example, ceramide modulates protein phosphorylation, the activity of protein kinase C (PKC), and phospholipase A2, and mediates signal transduction  ( 2) ( 3), while sphingosine and psychosine are potent inhibitors of PKC  ( 4).	transcription
67872	4	336146	7	NULL	NULL	0	NULL	ceramide	Chemical		mediates					signal transduction	Process				NULL		0	NULL	NULL	NULL	gw60_jlipidres_42_2_301_s_18	11181761	For example, ceramide modulates protein phosphorylation, the activity of protein kinase C (PKC), and phospholipase A2, and mediates signal transduction  ( 2) ( 3), while sphingosine and psychosine are potent inhibitors of PKC  ( 4).	transcription
67873	5	336146	7	NULL	NULL	0	NULL	sphingosine	Chemical		potent inhibitor of					PKC	GP				NULL		0	NULL	NULL	NULL	gw60_jlipidres_42_2_301_s_18	11181761	For example, ceramide modulates protein phosphorylation, the activity of protein kinase C (PKC), and phospholipase A2, and mediates signal transduction  ( 2) ( 3), while sphingosine and psychosine are potent inhibitors of PKC  ( 4).	transcription
67874	6	336146	7	NULL	NULL	0	NULL	psychosine	Chemical		potent inhibitor of					PKC	GP				NULL		0	NULL	NULL	NULL	gw60_jlipidres_42_2_301_s_18	11181761	For example, ceramide modulates protein phosphorylation, the activity of protein kinase C (PKC), and phospholipase A2, and mediates signal transduction  ( 2) ( 3), while sphingosine and psychosine are potent inhibitors of PKC  ( 4).	transcription
67875	7	336146	7	NULL	NULL	0	NULL	PKC	GP		is					protein kinase C	GP				NULL		0	NULL	NULL	NULL	gw60_jlipidres_42_2_301_s_18	11181761	For example, ceramide modulates protein phosphorylation, the activity of protein kinase C (PKC), and phospholipase A2, and mediates signal transduction  ( 2) ( 3), while sphingosine and psychosine are potent inhibitors of PKC  ( 4).	transcription
66946	1	336147	5	NULL	NULL	0	NULL	sphingomyelinases	GP		is activated by					TNF-alpha	GP				NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_17_7458_s_15	10460252	Activation of sphingomyelinases (SMases) by extracellular factors such as tumor necrosis factor-alpha (TNF-alpha) or Fas ligand leads to the formation of ceramide (cer), sphingosine (sph), and sphingosine-1-phosphate (SPP).	transcription
66947	2	336147	5	NULL	NULL	0	NULL	sphingomyelinases	GP		is activated by					Fas ligand	GP				NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_17_7458_s_15	10460252	Activation of sphingomyelinases (SMases) by extracellular factors such as tumor necrosis factor-alpha (TNF-alpha) or Fas ligand leads to the formation of ceramide (cer), sphingosine (sph), and sphingosine-1-phosphate (SPP).	transcription
66948	3	336147	5	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_17_7458_s_15	10460252	Activation of sphingomyelinases (SMases) by extracellular factors such as tumor necrosis factor-alpha (TNF-alpha) or Fas ligand leads to the formation of ceramide (cer), sphingosine (sph), and sphingosine-1-phosphate (SPP).	transcription
66949	4	336147	5	NULL	NULL	0	NULL	statement 1	Process		leads to					ceramide	Chemical	formation of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_17_7458_s_15	10460252	Activation of sphingomyelinases (SMases) by extracellular factors such as tumor necrosis factor-alpha (TNF-alpha) or Fas ligand leads to the formation of ceramide (cer), sphingosine (sph), and sphingosine-1-phosphate (SPP).	transcription
66950	5	336147	5	NULL	NULL	0	NULL	statement 2	Process		leads to					ceramide	Chemical	formation of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_17_7458_s_15	10460252	Activation of sphingomyelinases (SMases) by extracellular factors such as tumor necrosis factor-alpha (TNF-alpha) or Fas ligand leads to the formation of ceramide (cer), sphingosine (sph), and sphingosine-1-phosphate (SPP).	transcription
66951	6	336147	5	NULL	NULL	0	NULL	statement 1	Process		leads to					sphingosine	Chemical	formation of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_17_7458_s_15	10460252	Activation of sphingomyelinases (SMases) by extracellular factors such as tumor necrosis factor-alpha (TNF-alpha) or Fas ligand leads to the formation of ceramide (cer), sphingosine (sph), and sphingosine-1-phosphate (SPP).	transcription
66952	7	336147	5	NULL	NULL	0	NULL	statement 2	Process		leads to					sphingosine	Chemical	formation of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_17_7458_s_15	10460252	Activation of sphingomyelinases (SMases) by extracellular factors such as tumor necrosis factor-alpha (TNF-alpha) or Fas ligand leads to the formation of ceramide (cer), sphingosine (sph), and sphingosine-1-phosphate (SPP).	transcription
66953	8	336147	5	NULL	NULL	0	NULL	statement 1	Process		leads to					sphingosine 1-phosphate	Chemical	formation of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_17_7458_s_15	10460252	Activation of sphingomyelinases (SMases) by extracellular factors such as tumor necrosis factor-alpha (TNF-alpha) or Fas ligand leads to the formation of ceramide (cer), sphingosine (sph), and sphingosine-1-phosphate (SPP).	transcription
66954	9	336147	5	NULL	NULL	0	NULL	statement 2	Process		leads to					sphingosine 1-phosphate	Chemical	formation of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_17_7458_s_15	10460252	Activation of sphingomyelinases (SMases) by extracellular factors such as tumor necrosis factor-alpha (TNF-alpha) or Fas ligand leads to the formation of ceramide (cer), sphingosine (sph), and sphingosine-1-phosphate (SPP).	transcription
66955	10	336147	5	NULL	NULL	0	NULL	sphingomyelinases	GP		is					SMases	GP				NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_17_7458_s_15	10460252	Activation of sphingomyelinases (SMases) by extracellular factors such as tumor necrosis factor-alpha (TNF-alpha) or Fas ligand leads to the formation of ceramide (cer), sphingosine (sph), and sphingosine-1-phosphate (SPP).	transcription
66956	11	336147	5	NULL	NULL	0	NULL	TNF-alpha	GP		is					tumor necrosis factor-alpha	GP				NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_17_7458_s_15	10460252	Activation of sphingomyelinases (SMases) by extracellular factors such as tumor necrosis factor-alpha (TNF-alpha) or Fas ligand leads to the formation of ceramide (cer), sphingosine (sph), and sphingosine-1-phosphate (SPP).	transcription
66957	12	336147	5	NULL	NULL	0	NULL	ceramide	Chemical		is					cer	Chemical				NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_17_7458_s_15	10460252	Activation of sphingomyelinases (SMases) by extracellular factors such as tumor necrosis factor-alpha (TNF-alpha) or Fas ligand leads to the formation of ceramide (cer), sphingosine (sph), and sphingosine-1-phosphate (SPP).	transcription
66958	13	336147	5	NULL	NULL	0	NULL	sphingosine	Chemical		is					sph	Chemical				NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_17_7458_s_15	10460252	Activation of sphingomyelinases (SMases) by extracellular factors such as tumor necrosis factor-alpha (TNF-alpha) or Fas ligand leads to the formation of ceramide (cer), sphingosine (sph), and sphingosine-1-phosphate (SPP).	transcription
66959	14	336147	5	NULL	NULL	0	NULL	sphingosine 1-phosphate	Chemical		is					SPP	Chemical				NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_17_7458_s_15	10460252	Activation of sphingomyelinases (SMases) by extracellular factors such as tumor necrosis factor-alpha (TNF-alpha) or Fas ligand leads to the formation of ceramide (cer), sphingosine (sph), and sphingosine-1-phosphate (SPP).	transcription
67876	1	336147	7	NULL	NULL	0	NULL	TNF-alpha	GP		activates					SMases	GP				NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_17_7458_s_15	10460252	Activation of sphingomyelinases (SMases) by extracellular factors such as tumor necrosis factor-alpha (TNF-alpha) or Fas ligand leads to the formation of ceramide (cer), sphingosine (sph), and sphingosine-1-phosphate (SPP).	transcription
67877	2	336147	7	NULL	NULL	NULL	NULL	Fas ligand	GP		leads to					cer	Chemical	formation of			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_19_17_7458_s_15	10460252	Activation of sphingomyelinases (SMases) by extracellular factors such as tumor necrosis factor-alpha (TNF-alpha) or Fas ligand leads to the formation of ceramide (cer), sphingosine (sph), and sphingosine-1-phosphate (SPP).	transcription
67878	3	336147	7	NULL	NULL	NULL	NULL	Fas ligand	GP		leads to					sph	Chemical	formation of			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_19_17_7458_s_15	10460252	Activation of sphingomyelinases (SMases) by extracellular factors such as tumor necrosis factor-alpha (TNF-alpha) or Fas ligand leads to the formation of ceramide (cer), sphingosine (sph), and sphingosine-1-phosphate (SPP).	transcription
67879	4	336147	7	NULL	NULL	0	NULL	Fas ligand	GP		leads to					SPP	Chemical	formation of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_17_7458_s_15	10460252	Activation of sphingomyelinases (SMases) by extracellular factors such as tumor necrosis factor-alpha (TNF-alpha) or Fas ligand leads to the formation of ceramide (cer), sphingosine (sph), and sphingosine-1-phosphate (SPP).	transcription
67880	5	336147	7	NULL	NULL	0	NULL	SMases	GP		is					sphingomyelinases 	GP				NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_17_7458_s_15	10460252	Activation of sphingomyelinases (SMases) by extracellular factors such as tumor necrosis factor-alpha (TNF-alpha) or Fas ligand leads to the formation of ceramide (cer), sphingosine (sph), and sphingosine-1-phosphate (SPP).	transcription
67881	6	336147	7	NULL	NULL	0	NULL	TNF-alpha	GP		is					tumor necrosis factor-alpha	GP				NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_17_7458_s_15	10460252	Activation of sphingomyelinases (SMases) by extracellular factors such as tumor necrosis factor-alpha (TNF-alpha) or Fas ligand leads to the formation of ceramide (cer), sphingosine (sph), and sphingosine-1-phosphate (SPP).	transcription
67882	7	336147	7	NULL	NULL	0	NULL	cer	Chemical		is					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_17_7458_s_15	10460252	Activation of sphingomyelinases (SMases) by extracellular factors such as tumor necrosis factor-alpha (TNF-alpha) or Fas ligand leads to the formation of ceramide (cer), sphingosine (sph), and sphingosine-1-phosphate (SPP).	transcription
67883	8	336147	7	NULL	NULL	0	NULL	sph	Chemical		is					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_17_7458_s_15	10460252	Activation of sphingomyelinases (SMases) by extracellular factors such as tumor necrosis factor-alpha (TNF-alpha) or Fas ligand leads to the formation of ceramide (cer), sphingosine (sph), and sphingosine-1-phosphate (SPP).	transcription
67884	9	336147	7	NULL	NULL	0	NULL	SPP	Chemical		is					sphingosine-1-phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_17_7458_s_15	10460252	Activation of sphingomyelinases (SMases) by extracellular factors such as tumor necrosis factor-alpha (TNF-alpha) or Fas ligand leads to the formation of ceramide (cer), sphingosine (sph), and sphingosine-1-phosphate (SPP).	transcription
67885	10	336147	7	NULL	NULL	0	NULL	TNF-alpha	GP		is a type of					extracellular factor	GP				NULL		0	NULL	NULL	NULL	gw60_jneurosci_19_17_7458_s_15	10460252	Activation of sphingomyelinases (SMases) by extracellular factors such as tumor necrosis factor-alpha (TNF-alpha) or Fas ligand leads to the formation of ceramide (cer), sphingosine (sph), and sphingosine-1-phosphate (SPP).	transcription
66960	1	336148	5	NULL	NULL	0	NULL	programmed cell death	Process		is mediated by					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_236	9278531	Cuvillier O, Pirianov G, Kleuser B, Vanek P, Coso O, Gutkind J, Spiegel S    (1996) Sphingosine 1-phosphate inhibits ceramide mediated programmed cell death.	transcription
66961	2	336148	5	NULL	NULL	0	NULL	sphingosine 1-phosphate	Chemical		inhibits					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_236	9278531	Cuvillier O, Pirianov G, Kleuser B, Vanek P, Coso O, Gutkind J, Spiegel S    (1996) Sphingosine 1-phosphate inhibits ceramide mediated programmed cell death.	transcription
67886	1	336148	7	NULL	NULL	0	NULL	ceramide	Chemical		mediates					programmed cell death	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_236	9278531	Cuvillier O, Pirianov G, Kleuser B, Vanek P, Coso O, Gutkind J, Spiegel S    (1996) Sphingosine 1-phosphate inhibits ceramide mediated programmed cell death.	transcription
67887	2	336148	7	NULL	NULL	0	NULL	Sphingosine 1-phosphate	Chemical		inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_236	9278531	Cuvillier O, Pirianov G, Kleuser B, Vanek P, Coso O, Gutkind J, Spiegel S    (1996) Sphingosine 1-phosphate inhibits ceramide mediated programmed cell death.	transcription
66962	1	336149	5	NULL	NULL	0	NULL	programmed cell death	Process		is mediated by					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_9_2929_s_339	11312276	Guvillier O, Pirianov G, Kleuser B, Vanek PG, Coso OA, Gutkind JS, Spiegel S   (1996) Suppression of ceramide-mediated programmed cell death by sphingosine-a-phosphate.	transcription
66963	2	336149	5	NULL	NULL	0	NULL	sphingosine-a-phosphate	Chemical		suppress					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_9_2929_s_339	11312276	Guvillier O, Pirianov G, Kleuser B, Vanek PG, Coso OA, Gutkind JS, Spiegel S   (1996) Suppression of ceramide-mediated programmed cell death by sphingosine-a-phosphate.	transcription
67888	1	336149	7	NULL	NULL	0	NULL	ceramide	Chemical		mediate					programmed cell death	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_9_2929_s_339	11312276	Guvillier O, Pirianov G, Kleuser B, Vanek PG, Coso OA, Gutkind JS, Spiegel S   (1996) Suppression of ceramide-mediated programmed cell death by sphingosine-a-phosphate.	transcription
67889	2	336149	7	NULL	NULL	0	NULL	sphingosine-a-phosphate	Chemical		suppress					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_21_9_2929_s_339	11312276	Guvillier O, Pirianov G, Kleuser B, Vanek PG, Coso OA, Gutkind JS, Spiegel S   (1996) Suppression of ceramide-mediated programmed cell death by sphingosine-a-phosphate.	transcription
66964	1	336150	5	NULL	NULL	0	NULL	apoptosis	Process		is induced by					tumor necrosis factor-alpha	GP				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_184	10454518	For example, induction of apoptosis by tumor necrosis factor-alpha via activation of tumor necrosis factor R1 can involve acute generation of either ceramide (Jarvis et al., 1994a  ) or sphingosine (Ohta et al., 1994  ).	transcription
66965	2	336150	5	NULL	NULL	NULL	NULL	statement 1	Process		via					tumor necrosis factor R1	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_184	10454518	For example, induction of apoptosis by tumor necrosis factor-alpha via activation of tumor necrosis factor R1 can involve acute generation of either ceramide (Jarvis et al., 1994a  ) or sphingosine (Ohta et al., 1994  ).	transcription
66966	3	336150	5	NULL	NULL	0	NULL	statement 2	Process		involves					ceramide	Chemical	acute generation of			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_184	10454518	For example, induction of apoptosis by tumor necrosis factor-alpha via activation of tumor necrosis factor R1 can involve acute generation of either ceramide (Jarvis et al., 1994a  ) or sphingosine (Ohta et al., 1994  ).	transcription
66967	4	336150	5	NULL	NULL	0	NULL	statement 2	Process		involves					sphingosine	Chemical	acute generation of			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_184	10454518	For example, induction of apoptosis by tumor necrosis factor-alpha via activation of tumor necrosis factor R1 can involve acute generation of either ceramide (Jarvis et al., 1994a  ) or sphingosine (Ohta et al., 1994  ).	transcription
66968	5	336150	5	NULL	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_184	10454518	For example, induction of apoptosis by tumor necrosis factor-alpha via activation of tumor necrosis factor R1 can involve acute generation of either ceramide (Jarvis et al., 1994a  ) or sphingosine (Ohta et al., 1994  ).	transcription
67890	1	336150	7	NULL	NULL	0	NULL	tumor necrosis factor-alpha	GP		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_184	10454518	For example, induction of apoptosis by tumor necrosis factor-alpha via activation of tumor necrosis factor R1 can involve acute generation of either ceramide (Jarvis et al., 1994a  ) or sphingosine (Ohta et al., 1994  ).	transcription
67891	2	336150	7	NULL	NULL	0	NULL	statement 1	Process		via					R1	GP				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_184	10454518	For example, induction of apoptosis by tumor necrosis factor-alpha via activation of tumor necrosis factor R1 can involve acute generation of either ceramide (Jarvis et al., 1994a  ) or sphingosine (Ohta et al., 1994  ).	transcription
67892	3	336150	7	NULL	NULL	0	NULL	statement 1	Process		involve					ceramide	Chemical	acute generation of			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_184	10454518	For example, induction of apoptosis by tumor necrosis factor-alpha via activation of tumor necrosis factor R1 can involve acute generation of either ceramide (Jarvis et al., 1994a  ) or sphingosine (Ohta et al., 1994  ).	transcription
67893	4	336150	7	NULL	NULL	0	NULL	statement 1	Process		involve					sphingosine	Chemical	acute generation of			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_184	10454518	For example, induction of apoptosis by tumor necrosis factor-alpha via activation of tumor necrosis factor R1 can involve acute generation of either ceramide (Jarvis et al., 1994a  ) or sphingosine (Ohta et al., 1994  ).	transcription
67894	5	336150	7	NULL	NULL	0	NULL	R1	GP		is a type of					tumor necrosis factor	GP				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_184	10454518	For example, induction of apoptosis by tumor necrosis factor-alpha via activation of tumor necrosis factor R1 can involve acute generation of either ceramide (Jarvis et al., 1994a  ) or sphingosine (Ohta et al., 1994  ).	transcription
66969	1	336151	5	NULL	NULL	NULL	NULL	dihydro-C2-ceramide	Chemical		does not inhibit		significantly			n-K+ channels	GP				NULL	JCaM1.6 cells	NULL	NULL	NULL	NULL	gw60_pnas_94_14_7661_s_108	9207149	Furthermore, dihydro-C2-ceramide or sphingosine did not significantly inhibit n-K+ channels in JCaM1.6 or herbimycin A-treated cells, excluding a direct, structural inhibition of n-K+ channels by ceramide.	transcription
66970	2	336151	5	NULL	NULL	0	NULL	sphingosine	Chemical		does not inhibit		significantly			n-K+ channels	GP				NULL	JCaM1.6 cells	0	NULL	NULL	NULL	gw60_pnas_94_14_7661_s_108	9207149	Furthermore, dihydro-C2-ceramide or sphingosine did not significantly inhibit n-K+ channels in JCaM1.6 or herbimycin A-treated cells, excluding a direct, structural inhibition of n-K+ channels by ceramide.	transcription
66971	3	336151	5	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_94_14_7661_s_108	9207149	Furthermore, dihydro-C2-ceramide or sphingosine did not significantly inhibit n-K+ channels in JCaM1.6 or herbimycin A-treated cells, excluding a direct, structural inhibition of n-K+ channels by ceramide.	transcription
66972	4	336151	5	NULL	NULL	0	NULL	dihydro-C2-ceramide	Chemical		does not inhibit		significantly			n-K+ channels	GP				NULL	herbimycin A-treated cells	0	NULL	NULL	NULL	gw60_pnas_94_14_7661_s_108	9207149	Furthermore, dihydro-C2-ceramide or sphingosine did not significantly inhibit n-K+ channels in JCaM1.6 or herbimycin A-treated cells, excluding a direct, structural inhibition of n-K+ channels by ceramide.	transcription
66973	5	336151	5	NULL	NULL	0	NULL	sphingosine	Chemical		does not inhibit		significantly			n-K+ channels	GP				NULL	herbimycin A-treated cells	0	NULL	NULL	NULL	gw60_pnas_94_14_7661_s_108	9207149	Furthermore, dihydro-C2-ceramide or sphingosine did not significantly inhibit n-K+ channels in JCaM1.6 or herbimycin A-treated cells, excluding a direct, structural inhibition of n-K+ channels by ceramide.	transcription
66974	6	336151	5	NULL	NULL	0	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_94_14_7661_s_108	9207149	Furthermore, dihydro-C2-ceramide or sphingosine did not significantly inhibit n-K+ channels in JCaM1.6 or herbimycin A-treated cells, excluding a direct, structural inhibition of n-K+ channels by ceramide.	transcription
66975	7	336151	5	NULL	NULL	NULL	NULL	ceramide	Chemical		inhibits		direct;;structural			n-K+ channels	GP				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_14_7661_s_108	9207149	Furthermore, dihydro-C2-ceramide or sphingosine did not significantly inhibit n-K+ channels in JCaM1.6 or herbimycin A-treated cells, excluding a direct, structural inhibition of n-K+ channels by ceramide.	transcription
66976	8	336151	5	NULL	NULL	0	NULL	statement 1	Process		exclude					statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_94_14_7661_s_108	9207149	Furthermore, dihydro-C2-ceramide or sphingosine did not significantly inhibit n-K+ channels in JCaM1.6 or herbimycin A-treated cells, excluding a direct, structural inhibition of n-K+ channels by ceramide.	transcription
66977	9	336151	5	NULL	NULL	0	NULL	statement 2	Process		exclude					statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_94_14_7661_s_108	9207149	Furthermore, dihydro-C2-ceramide or sphingosine did not significantly inhibit n-K+ channels in JCaM1.6 or herbimycin A-treated cells, excluding a direct, structural inhibition of n-K+ channels by ceramide.	transcription
66978	10	336151	5	NULL	NULL	0	NULL	statement 4	Process		exclude					statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_94_14_7661_s_108	9207149	Furthermore, dihydro-C2-ceramide or sphingosine did not significantly inhibit n-K+ channels in JCaM1.6 or herbimycin A-treated cells, excluding a direct, structural inhibition of n-K+ channels by ceramide.	transcription
66979	11	336151	5	NULL	NULL	0	NULL	statement 5	Process		exclude					statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_94_14_7661_s_108	9207149	Furthermore, dihydro-C2-ceramide or sphingosine did not significantly inhibit n-K+ channels in JCaM1.6 or herbimycin A-treated cells, excluding a direct, structural inhibition of n-K+ channels by ceramide.	transcription
69437	1	336151	7	NULL	NULL	0	NULL	dihydro-C2-ceramide	Chemical		does not inhibit		significantly			n-K+ channels	Chemical				NULL	JCaM1.6 treated cells	0	NULL	NULL	NULL	gw60_pnas_94_14_7661_s_108	9207149	Furthermore, dihydro-C2-ceramide or sphingosine did not significantly inhibit n-K+ channels in JCaM1.6 or herbimycin A-treated cells, excluding a direct, structural inhibition of n-K+ channels by ceramide.	transcription
69438	2	336151	7	NULL	NULL	0	NULL	 dihydro-C2-ceramide	Chemical		does not inhibit		significantly			n-K+ channels	Chemical				NULL	herbimycin A-treated cells	0	NULL	NULL	NULL	gw60_pnas_94_14_7661_s_108	9207149	Furthermore, dihydro-C2-ceramide or sphingosine did not significantly inhibit n-K+ channels in JCaM1.6 or herbimycin A-treated cells, excluding a direct, structural inhibition of n-K+ channels by ceramide.	transcription
69439	3	336151	7	NULL	NULL	0	NULL	sphingosine	Chemical		does not inhibit		significantly			n-K+ channels	Chemical				NULL	JCaM1.6 treated cells	0	NULL	NULL	NULL	gw60_pnas_94_14_7661_s_108	9207149	Furthermore, dihydro-C2-ceramide or sphingosine did not significantly inhibit n-K+ channels in JCaM1.6 or herbimycin A-treated cells, excluding a direct, structural inhibition of n-K+ channels by ceramide.	transcription
69440	4	336151	7	NULL	NULL	0	NULL	sphingosine	Chemical		does not inhibit		significantly			n-K+ channels	Chemical				NULL	herbimycin A-treated cells	0	NULL	NULL	NULL	gw60_pnas_94_14_7661_s_108	9207149	Furthermore, dihydro-C2-ceramide or sphingosine did not significantly inhibit n-K+ channels in JCaM1.6 or herbimycin A-treated cells, excluding a direct, structural inhibition of n-K+ channels by ceramide.	transcription
69441	5	336151	7	NULL	NULL	0	NULL	ceramide	Chemical		inhibit		direct;;structurally			n-K+ channels 	Chemical				NULL		0	NULL	NULL	NULL	gw60_pnas_94_14_7661_s_108	9207149	Furthermore, dihydro-C2-ceramide or sphingosine did not significantly inhibit n-K+ channels in JCaM1.6 or herbimycin A-treated cells, excluding a direct, structural inhibition of n-K+ channels by ceramide.	transcription
66980	1	336152	5	NULL	NULL	0	NULL	sphingosine-recycling pathway	Process		generates					long-chain ceramide	Chemical	endogenous			NULL		0	NULL	NULL	NULL	abs-batch0550-0559_biochem-j_393_pt-2_16201965_s_10	16201965	These  data demonstrate that the sphingosine-recycling pathway for the generation  of endogenous long-chain ceramide in response to exogenous C(6)-cer is  regulated by ROS, and plays an important biological role in controlling  c-Myc function.	transcription
66981	2	336152	5	NULL	NULL	0	NULL	statement 1	Process		in response to					C(6)-cer	Chemical	exogenous			NULL		0	NULL	NULL	NULL	abs-batch0550-0559_biochem-j_393_pt-2_16201965_s_10	16201965	These  data demonstrate that the sphingosine-recycling pathway for the generation  of endogenous long-chain ceramide in response to exogenous C(6)-cer is  regulated by ROS, and plays an important biological role in controlling  c-Myc function.	transcription
66982	3	336152	5	NULL	NULL	0	NULL	statement 2	Process		is regulated by					ROS	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0550-0559_biochem-j_393_pt-2_16201965_s_10	16201965	These  data demonstrate that the sphingosine-recycling pathway for the generation  of endogenous long-chain ceramide in response to exogenous C(6)-cer is  regulated by ROS, and plays an important biological role in controlling  c-Myc function.	transcription
66983	4	336152	5	NULL	NULL	0	NULL	statement 1	Process		plays a role in		biological			c-Myc	GP	controlling;;function of			NULL		0	NULL	NULL	NULL	abs-batch0550-0559_biochem-j_393_pt-2_16201965_s_10	16201965	These  data demonstrate that the sphingosine-recycling pathway for the generation  of endogenous long-chain ceramide in response to exogenous C(6)-cer is  regulated by ROS, and plays an important biological role in controlling  c-Myc function.	transcription
69442	1	336152	7	NULL	NULL	0	NULL	 C(6)-cer	Chemical	exogenous	generate					long-chain ceramide	Chemical	endogenous			NULL		0	NULL	NULL	NULL	abs-batch0550-0559_biochem-j_393_pt-2_16201965_s_10	16201965	These  data demonstrate that the sphingosine-recycling pathway for the generation  of endogenous long-chain ceramide in response to exogenous C(6)-cer is  regulated by ROS, and plays an important biological role in controlling  c-Myc function.	transcription
69443	2	336152	7	NULL	NULL	0	NULL	ROS	Chemical		regulate					statement 1	Process				NULL		0	NULL	NULL	NULL	abs-batch0550-0559_biochem-j_393_pt-2_16201965_s_10	16201965	These  data demonstrate that the sphingosine-recycling pathway for the generation  of endogenous long-chain ceramide in response to exogenous C(6)-cer is  regulated by ROS, and plays an important biological role in controlling  c-Myc function.	transcription
69444	3	336152	7	NULL	NULL	0	NULL	statement 2	Process		play a role in		important			c-Myc	GP	function of			NULL		0	NULL	NULL	NULL	abs-batch0550-0559_biochem-j_393_pt-2_16201965_s_10	16201965	These  data demonstrate that the sphingosine-recycling pathway for the generation  of endogenous long-chain ceramide in response to exogenous C(6)-cer is  regulated by ROS, and plays an important biological role in controlling  c-Myc function.	transcription
69445	4	336152	7	NULL	NULL	0	NULL	statement 1	Process		is a type of					sphingosine-recycling pathway	Process				NULL		0	NULL	NULL	NULL	abs-batch0550-0559_biochem-j_393_pt-2_16201965_s_10	16201965	These  data demonstrate that the sphingosine-recycling pathway for the generation  of endogenous long-chain ceramide in response to exogenous C(6)-cer is  regulated by ROS, and plays an important biological role in controlling  c-Myc function.	transcription
66984	1	336153	5	NULL	NULL	0	NULL	ceramide	Chemical		causes					apoptosis	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biochem-mol-biol_39_2_16584625_s_3	16584625	The balance between cellular levels of these  bioactive products is increasingly recognized to be critical to cell regulation;  whereby, ceramide and sphingosine cause apoptosis and growth arrest phenotypes,  and sphingosine-1-phosphate mediates proliferative and angiogenic responses.	transcription
66985	2	336153	5	NULL	NULL	0	NULL	sphingosine	Chemical		causes					apoptosis	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biochem-mol-biol_39_2_16584625_s_3	16584625	The balance between cellular levels of these  bioactive products is increasingly recognized to be critical to cell regulation;  whereby, ceramide and sphingosine cause apoptosis and growth arrest phenotypes,  and sphingosine-1-phosphate mediates proliferative and angiogenic responses.	transcription
66986	3	336153	5	NULL	NULL	0	NULL	ceramide	Chemical		causes					growth arrest phenotypes					NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biochem-mol-biol_39_2_16584625_s_3	16584625	The balance between cellular levels of these  bioactive products is increasingly recognized to be critical to cell regulation;  whereby, ceramide and sphingosine cause apoptosis and growth arrest phenotypes,  and sphingosine-1-phosphate mediates proliferative and angiogenic responses.	transcription
66987	4	336153	5	NULL	NULL	0	NULL	sphingosine	Chemical		causes					growth arrest phenotypes					NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biochem-mol-biol_39_2_16584625_s_3	16584625	The balance between cellular levels of these  bioactive products is increasingly recognized to be critical to cell regulation;  whereby, ceramide and sphingosine cause apoptosis and growth arrest phenotypes,  and sphingosine-1-phosphate mediates proliferative and angiogenic responses.	transcription
66988	5	336153	5	NULL	NULL	0	NULL	sphingosine 1-phosphate	Chemical		mediates					proliferative responses	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biochem-mol-biol_39_2_16584625_s_3	16584625	The balance between cellular levels of these  bioactive products is increasingly recognized to be critical to cell regulation;  whereby, ceramide and sphingosine cause apoptosis and growth arrest phenotypes,  and sphingosine-1-phosphate mediates proliferative and angiogenic responses.	transcription
66989	6	336153	5	NULL	NULL	0	NULL	sphingosine 1-phosphate	Chemical		mediates					angiogenic responses	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biochem-mol-biol_39_2_16584625_s_3	16584625	The balance between cellular levels of these  bioactive products is increasingly recognized to be critical to cell regulation;  whereby, ceramide and sphingosine cause apoptosis and growth arrest phenotypes,  and sphingosine-1-phosphate mediates proliferative and angiogenic responses.	transcription
69446	1	336153	7	NULL	NULL	0	NULL	ceramide	Chemical		cause					apoptosis	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biochem-mol-biol_39_2_16584625_s_3	16584625	The balance between cellular levels of these  bioactive products is increasingly recognized to be critical to cell regulation;  whereby, ceramide and sphingosine cause apoptosis and growth arrest phenotypes,  and sphingosine-1-phosphate mediates proliferative and angiogenic responses.	transcription
69447	2	336153	7	NULL	NULL	0	NULL	sphingosine	Chemical		cause					apoptosis	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biochem-mol-biol_39_2_16584625_s_3	16584625	The balance between cellular levels of these  bioactive products is increasingly recognized to be critical to cell regulation;  whereby, ceramide and sphingosine cause apoptosis and growth arrest phenotypes,  and sphingosine-1-phosphate mediates proliferative and angiogenic responses.	transcription
69448	3	336153	7	NULL	NULL	0	NULL	ceramide	Chemical		cause					growth arrest phenotypes	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biochem-mol-biol_39_2_16584625_s_3	16584625	The balance between cellular levels of these  bioactive products is increasingly recognized to be critical to cell regulation;  whereby, ceramide and sphingosine cause apoptosis and growth arrest phenotypes,  and sphingosine-1-phosphate mediates proliferative and angiogenic responses.	transcription
69449	4	336153	7	NULL	NULL	0	NULL	sphingosine	Chemical		cause					growth arrest phenotypes	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biochem-mol-biol_39_2_16584625_s_3	16584625	The balance between cellular levels of these  bioactive products is increasingly recognized to be critical to cell regulation;  whereby, ceramide and sphingosine cause apoptosis and growth arrest phenotypes,  and sphingosine-1-phosphate mediates proliferative and angiogenic responses.	transcription
69450	5	336153	7	NULL	NULL	0	NULL	sphingosine-1-phosphate	Chemical		mediates					proliferative response	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biochem-mol-biol_39_2_16584625_s_3	16584625	The balance between cellular levels of these  bioactive products is increasingly recognized to be critical to cell regulation;  whereby, ceramide and sphingosine cause apoptosis and growth arrest phenotypes,  and sphingosine-1-phosphate mediates proliferative and angiogenic responses.	transcription
69451	6	336153	7	NULL	NULL	0	NULL	sphingosine-1-phosphate	Chemical		mediates					angiogenic response	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biochem-mol-biol_39_2_16584625_s_3	16584625	The balance between cellular levels of these  bioactive products is increasingly recognized to be critical to cell regulation;  whereby, ceramide and sphingosine cause apoptosis and growth arrest phenotypes,  and sphingosine-1-phosphate mediates proliferative and angiogenic responses.	transcription
66990	1	336154	5	NULL	NULL	0	NULL	apoptosis	Process		is induced by					TNF-alpha	GP				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_cytokine_34_1-2_16730193_s_3	16730193	Sphingosine/ceramide  and nitric oxide have been associated with apoptosis induced by TNF-alpha;  however, signaling mechanisms of TNF-alpha-induced apoptosis in cardiac  myocytes are not well defined.	transcription
66991	2	336154	5	NULL	NULL	0	NULL	sphingosine/ceramide	Chemical		is associated with					statement 1	Process				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_cytokine_34_1-2_16730193_s_3	16730193	Sphingosine/ceramide  and nitric oxide have been associated with apoptosis induced by TNF-alpha;  however, signaling mechanisms of TNF-alpha-induced apoptosis in cardiac  myocytes are not well defined.	transcription
66992	3	336154	5	NULL	NULL	0	NULL	nitric oxide	Chemical		is associated with					statement 1	Process				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_cytokine_34_1-2_16730193_s_3	16730193	Sphingosine/ceramide  and nitric oxide have been associated with apoptosis induced by TNF-alpha;  however, signaling mechanisms of TNF-alpha-induced apoptosis in cardiac  myocytes are not well defined.	transcription
66993	4	336154	5	NULL	NULL	0	NULL	apoptosis	Process		is induced by					TNF-alpha	GP				NULL	cardiac myocytes	0	NULL	NULL	NULL	abs-batch0700-0719_cytokine_34_1-2_16730193_s_3	16730193	Sphingosine/ceramide  and nitric oxide have been associated with apoptosis induced by TNF-alpha;  however, signaling mechanisms of TNF-alpha-induced apoptosis in cardiac  myocytes are not well defined.	transcription
69452	1	336154	7	NULL	NULL	0	NULL	TNF-alpha	GP		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_cytokine_34_1-2_16730193_s_3	16730193	Sphingosine/ceramide  and nitric oxide have been associated with apoptosis induced by TNF-alpha;  however, signaling mechanisms of TNF-alpha-induced apoptosis in cardiac  myocytes are not well defined.	transcription
69453	2	336154	7	NULL	NULL	0	NULL	Sphingosine	Chemical		associated with					statement 1	Process				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_cytokine_34_1-2_16730193_s_3	16730193	Sphingosine/ceramide  and nitric oxide have been associated with apoptosis induced by TNF-alpha;  however, signaling mechanisms of TNF-alpha-induced apoptosis in cardiac  myocytes are not well defined.	transcription
69454	3	336154	7	NULL	NULL	0	NULL	ceramide	Chemical		associated with					statement 1	Process				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_cytokine_34_1-2_16730193_s_3	16730193	Sphingosine/ceramide  and nitric oxide have been associated with apoptosis induced by TNF-alpha;  however, signaling mechanisms of TNF-alpha-induced apoptosis in cardiac  myocytes are not well defined.	transcription
69455	4	336154	7	NULL	NULL	0	NULL	 nitric oxide	Chemical		associated with					statement 1	Process				NULL		0	NULL	NULL	NULL	abs-batch0700-0719_cytokine_34_1-2_16730193_s_3	16730193	Sphingosine/ceramide  and nitric oxide have been associated with apoptosis induced by TNF-alpha;  however, signaling mechanisms of TNF-alpha-induced apoptosis in cardiac  myocytes are not well defined.	transcription
69456	5	336154	7	NULL	NULL	0	NULL	TNF-alpha	GP		induce					apoptosis	Process				NULL	cardiac myocytes	0	NULL	NULL	NULL	abs-batch0700-0719_cytokine_34_1-2_16730193_s_3	16730193	Sphingosine/ceramide  and nitric oxide have been associated with apoptosis induced by TNF-alpha;  however, signaling mechanisms of TNF-alpha-induced apoptosis in cardiac  myocytes are not well defined.	transcription
66994	1	336155	5	NULL	NULL	0	NULL	PLD	GP		is					phospholipase D	GP				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochim-biophys-acta_1348_3_9366247_s_6	9366247	Moreover, in contrast to sphingosine which activates  phospholipase D (PLD) leading to an increase in phosphatidic acid levels,  sphingomyelinase, but not ceramide analogs, reduced TPA-stimulated PLD  activity.	transcription
66995	2	336155	5	NULL	NULL	0	NULL	sphingosine	Chemical		activates					PLD	GP				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochim-biophys-acta_1348_3_9366247_s_6	9366247	Moreover, in contrast to sphingosine which activates  phospholipase D (PLD) leading to an increase in phosphatidic acid levels,  sphingomyelinase, but not ceramide analogs, reduced TPA-stimulated PLD  activity.	transcription
66999	4	336155	5	NULL	NULL	NULL	NULL	PLD	GP	activity of	is stimulated by					TPA	Chemical				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_biochim-biophys-acta_1348_3_9366247_s_6	9366247	Moreover, in contrast to sphingosine which activates  phospholipase D (PLD) leading to an increase in phosphatidic acid levels,  sphingomyelinase, but not ceramide analogs, reduced TPA-stimulated PLD  activity.	transcription
67001	3	336155	5	NULL	NULL	0	NULL	statement 2	Process		increases					phosphatidic acid	Chemical	level of			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochim-biophys-acta_1348_3_9366247_s_6	9366247	Moreover, in contrast to sphingosine which activates  phospholipase D (PLD) leading to an increase in phosphatidic acid levels,  sphingomyelinase, but not ceramide analogs, reduced TPA-stimulated PLD  activity.	transcription
67002	5	336155	5	NULL	NULL	0	NULL	sphingomyelinase	GP		reduce					statement 4	Process				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochim-biophys-acta_1348_3_9366247_s_6	9366247	Moreover, in contrast to sphingosine which activates  phospholipase D (PLD) leading to an increase in phosphatidic acid levels,  sphingomyelinase, but not ceramide analogs, reduced TPA-stimulated PLD  activity.	transcription
67003	6	336155	5	NULL	NULL	0	NULL	ceramide analogs	Chemical		does not reduce					statement 4	Process				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochim-biophys-acta_1348_3_9366247_s_6	9366247	Moreover, in contrast to sphingosine which activates  phospholipase D (PLD) leading to an increase in phosphatidic acid levels,  sphingomyelinase, but not ceramide analogs, reduced TPA-stimulated PLD  activity.	transcription
69457	1	336155	7	NULL	NULL	0	NULL	sphingosine	Chemical		activates					PLD	GP				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochim-biophys-acta_1348_3_9366247_s_6	9366247	Moreover, in contrast to sphingosine which activates  phospholipase D (PLD) leading to an increase in phosphatidic acid levels,  sphingomyelinase, but not ceramide analogs, reduced TPA-stimulated PLD  activity.	transcription
69458	2	336155	7	NULL	NULL	0	NULL	statement 1	Process		increase					phosphatidic acid 	Chemical	levels of			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochim-biophys-acta_1348_3_9366247_s_6	9366247	Moreover, in contrast to sphingosine which activates  phospholipase D (PLD) leading to an increase in phosphatidic acid levels,  sphingomyelinase, but not ceramide analogs, reduced TPA-stimulated PLD  activity.	transcription
69459	3	336155	7	NULL	NULL	0	NULL	statement 1	Process		increase					sphingomyelinase	GP				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochim-biophys-acta_1348_3_9366247_s_6	9366247	Moreover, in contrast to sphingosine which activates  phospholipase D (PLD) leading to an increase in phosphatidic acid levels,  sphingomyelinase, but not ceramide analogs, reduced TPA-stimulated PLD  activity.	transcription
69460	4	336155	7	NULL	NULL	0	NULL	statement 1	Process		does not increase					ceramide analogs	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochim-biophys-acta_1348_3_9366247_s_6	9366247	Moreover, in contrast to sphingosine which activates  phospholipase D (PLD) leading to an increase in phosphatidic acid levels,  sphingomyelinase, but not ceramide analogs, reduced TPA-stimulated PLD  activity.	transcription
69461	5	336155	7	NULL	NULL	0	NULL	TPA	Chemical		stimulates					PLD	GP	activity of			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochim-biophys-acta_1348_3_9366247_s_6	9366247	Moreover, in contrast to sphingosine which activates  phospholipase D (PLD) leading to an increase in phosphatidic acid levels,  sphingomyelinase, but not ceramide analogs, reduced TPA-stimulated PLD  activity.	transcription
69462	6	336155	7	NULL	NULL	0	NULL	statement 1	Process		reduce					statement 5	Process				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochim-biophys-acta_1348_3_9366247_s_6	9366247	Moreover, in contrast to sphingosine which activates  phospholipase D (PLD) leading to an increase in phosphatidic acid levels,  sphingomyelinase, but not ceramide analogs, reduced TPA-stimulated PLD  activity.	transcription
69463	7	336155	7	NULL	NULL	0	NULL	PLD	GP		is					phospholipase D	GP				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_biochim-biophys-acta_1348_3_9366247_s_6	9366247	Moreover, in contrast to sphingosine which activates  phospholipase D (PLD) leading to an increase in phosphatidic acid levels,  sphingomyelinase, but not ceramide analogs, reduced TPA-stimulated PLD  activity.	transcription
67004	1	336156	5	NULL	NULL	0	NULL	phospholipase D	GP	stimulation of	increases					phosphatidic acid	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_chem-phys-lipids_80_1-2_8681426_s_6	8681426	Stimulation  of phospholipase D leading to an increase in phosphatidic acid, a positive  regulator of cell growth, by sphingosine and SPP, and its inhibition by  ceramide, might be related to their opposite effects on cell growth.	transcription
67005	2	336156	5	NULL	NULL	0	NULL	phosphatidic acid	Chemical		is a regulator of		positive			cell growth	Process				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_chem-phys-lipids_80_1-2_8681426_s_6	8681426	Stimulation  of phospholipase D leading to an increase in phosphatidic acid, a positive  regulator of cell growth, by sphingosine and SPP, and its inhibition by  ceramide, might be related to their opposite effects on cell growth.	transcription
67006	3	336156	5	NULL	NULL	0	NULL	sphingosine	Chemical		is required for					statement 1	Process				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_chem-phys-lipids_80_1-2_8681426_s_6	8681426	Stimulation  of phospholipase D leading to an increase in phosphatidic acid, a positive  regulator of cell growth, by sphingosine and SPP, and its inhibition by  ceramide, might be related to their opposite effects on cell growth.	transcription
67007	4	336156	5	NULL	NULL	0	NULL	SPP	Chemical		is required for					statement 1	Process				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_chem-phys-lipids_80_1-2_8681426_s_6	8681426	Stimulation  of phospholipase D leading to an increase in phosphatidic acid, a positive  regulator of cell growth, by sphingosine and SPP, and its inhibition by  ceramide, might be related to their opposite effects on cell growth.	transcription
67008	5	336156	5	NULL	NULL	0	NULL	ceramide	Chemical		inhibits					statement 1	Process				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_chem-phys-lipids_80_1-2_8681426_s_6	8681426	Stimulation  of phospholipase D leading to an increase in phosphatidic acid, a positive  regulator of cell growth, by sphingosine and SPP, and its inhibition by  ceramide, might be related to their opposite effects on cell growth.	transcription
71170	1	336156	7	NULL	NULL	NULL	NULL	phospholipase D	GP	stimulation of	leads to					phosphatidic acid	Chemical	increase in			NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_chem-phys-lipids_80_1-2_8681426_s_6	8681426	Stimulation  of phospholipase D leading to an increase in phosphatidic acid, a positive  regulator of cell growth, by sphingosine and SPP, and its inhibition by  ceramide, might be related to their opposite effects on cell growth.	transcription
71171	2	336156	7	NULL	NULL	NULL	NULL	phosphatidic acid	Chemical		 regulator of		 positive			cell growth	Process				NULL		NULL	NULL	NULL	NULL	abs-batch0720-0739_chem-phys-lipids_80_1-2_8681426_s_6	8681426	Stimulation  of phospholipase D leading to an increase in phosphatidic acid, a positive  regulator of cell growth, by sphingosine and SPP, and its inhibition by  ceramide, might be related to their opposite effects on cell growth.	transcription
71172	3	336156	7	NULL	NULL	0	NULL	sphingosine	Chemical		stimulate					phospholipase D	GP				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_chem-phys-lipids_80_1-2_8681426_s_6	8681426	Stimulation  of phospholipase D leading to an increase in phosphatidic acid, a positive  regulator of cell growth, by sphingosine and SPP, and its inhibition by  ceramide, might be related to their opposite effects on cell growth.	transcription
71173	4	336156	7	NULL	NULL	0	NULL	SPP	Chemical		stimulate					phospholipase D	GP				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_chem-phys-lipids_80_1-2_8681426_s_6	8681426	Stimulation  of phospholipase D leading to an increase in phosphatidic acid, a positive  regulator of cell growth, by sphingosine and SPP, and its inhibition by  ceramide, might be related to their opposite effects on cell growth.	transcription
71174	5	336156	7	NULL	NULL	0	NULL	ceramide	Chemical		inhibit					phospholipase D	GP				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_chem-phys-lipids_80_1-2_8681426_s_6	8681426	Stimulation  of phospholipase D leading to an increase in phosphatidic acid, a positive  regulator of cell growth, by sphingosine and SPP, and its inhibition by  ceramide, might be related to their opposite effects on cell growth.	transcription
71175	6	336156	7	NULL	NULL	0	NULL	statement 5	Process		cause					cell growth	Process	opposite effect on			NULL		0	NULL	NULL	NULL	abs-batch0720-0739_chem-phys-lipids_80_1-2_8681426_s_6	8681426	Stimulation  of phospholipase D leading to an increase in phosphatidic acid, a positive  regulator of cell growth, by sphingosine and SPP, and its inhibition by  ceramide, might be related to their opposite effects on cell growth.	transcription
67009	1	336157	5	NULL	NULL	NULL	NULL	promotive immune response	Process		is induced by					alpha-mannosyl ceramide analogues	Chemical				NULL	Valpha19 NKT cell	NULL	NULL	NULL	NULL	abs-batch0720-0739_eur-j-med-chem_41_5_16545892_s_1	16545892	Induction of promotive rather than suppressive immune responses from a novel NKT cell repertoire Valpha19 NKT cell with alpha-mannosyl ceramide analogues consisting of the immunosuppressant ISP-I as the sphingosine unit..	transcription
67010	2	336157	5	NULL	NULL	0	NULL	alpha-mannosyl ceramide analogues	Chemical		consists of					ISP-I	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_eur-j-med-chem_41_5_16545892_s_1	16545892	Induction of promotive rather than suppressive immune responses from a novel NKT cell repertoire Valpha19 NKT cell with alpha-mannosyl ceramide analogues consisting of the immunosuppressant ISP-I as the sphingosine unit..	transcription
67011	3	336157	5	NULL	NULL	0	NULL	ISP-I	Chemical		is a type of					immunosuppressant	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_eur-j-med-chem_41_5_16545892_s_1	16545892	Induction of promotive rather than suppressive immune responses from a novel NKT cell repertoire Valpha19 NKT cell with alpha-mannosyl ceramide analogues consisting of the immunosuppressant ISP-I as the sphingosine unit..	transcription
67012	4	336157	5	NULL	NULL	0	NULL	ISP-I	Chemical		is a unit of					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_eur-j-med-chem_41_5_16545892_s_1	16545892	Induction of promotive rather than suppressive immune responses from a novel NKT cell repertoire Valpha19 NKT cell with alpha-mannosyl ceramide analogues consisting of the immunosuppressant ISP-I as the sphingosine unit..	transcription
67013	5	336157	5	NULL	NULL	0	NULL	Valpha19 NKT cell	Cell		is repertoire of		novel			NKT cell	Cell				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_eur-j-med-chem_41_5_16545892_s_1	16545892	Induction of promotive rather than suppressive immune responses from a novel NKT cell repertoire Valpha19 NKT cell with alpha-mannosyl ceramide analogues consisting of the immunosuppressant ISP-I as the sphingosine unit..	transcription
67014	6	336157	5	NULL	NULL	NULL	NULL	suppressive immune response	Process		is not induced by					alpha-mannosyl ceramide analogues	Chemical				NULL	Valpha19 NKT cell	NULL	NULL	NULL	NULL	abs-batch0720-0739_eur-j-med-chem_41_5_16545892_s_1	16545892	Induction of promotive rather than suppressive immune responses from a novel NKT cell repertoire Valpha19 NKT cell with alpha-mannosyl ceramide analogues consisting of the immunosuppressant ISP-I as the sphingosine unit..	transcription
71176	1	336157	7	NULL	NULL	0	NULL	Valpha19 NKT cell 	Cell		consist of					alpha-mannosyl ceramide analogues	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_eur-j-med-chem_41_5_16545892_s_1	16545892	Induction of promotive rather than suppressive immune responses from a novel NKT cell repertoire Valpha19 NKT cell with alpha-mannosyl ceramide analogues consisting of the immunosuppressant ISP-I as the sphingosine unit..	transcription
71177	2	336157	7	NULL	NULL	0	NULL	alpha-mannosyl ceramide analogues	Chemical		consist of					ISP-I 	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_eur-j-med-chem_41_5_16545892_s_1	16545892	Induction of promotive rather than suppressive immune responses from a novel NKT cell repertoire Valpha19 NKT cell with alpha-mannosyl ceramide analogues consisting of the immunosuppressant ISP-I as the sphingosine unit..	transcription
71178	3	336157	7	NULL	NULL	0	NULL	ISP-I 	Chemical		is a type of					immunosuppressant	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_eur-j-med-chem_41_5_16545892_s_1	16545892	Induction of promotive rather than suppressive immune responses from a novel NKT cell repertoire Valpha19 NKT cell with alpha-mannosyl ceramide analogues consisting of the immunosuppressant ISP-I as the sphingosine unit..	transcription
71179	4	336157	7	NULL	NULL	0	NULL	ISP-I	Chemical		is a type of					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_eur-j-med-chem_41_5_16545892_s_1	16545892	Induction of promotive rather than suppressive immune responses from a novel NKT cell repertoire Valpha19 NKT cell with alpha-mannosyl ceramide analogues consisting of the immunosuppressant ISP-I as the sphingosine unit..	transcription
71180	5	336157	7	NULL	NULL	0	NULL	Valpha19 NKT cell	Cell		induce					promotive immune response	Process				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_eur-j-med-chem_41_5_16545892_s_1	16545892	Induction of promotive rather than suppressive immune responses from a novel NKT cell repertoire Valpha19 NKT cell with alpha-mannosyl ceramide analogues consisting of the immunosuppressant ISP-I as the sphingosine unit..	transcription
71181	6	336157	7	NULL	NULL	0	NULL	Valpha19 NKT cell	Cell		is a type of					novel NKT cell repertoire	Cell				NULL		0	NULL	NULL	NULL	abs-batch0720-0739_eur-j-med-chem_41_5_16545892_s_1	16545892	Induction of promotive rather than suppressive immune responses from a novel NKT cell repertoire Valpha19 NKT cell with alpha-mannosyl ceramide analogues consisting of the immunosuppressant ISP-I as the sphingosine unit..	transcription
67015	1	336158	5	NULL	NULL	0	NULL	sphingosine	Chemical	exogenous	increases					ceramide acyl chain species	Chemical	mass of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_44_37118_s_249	16118219	Exogenous sphingosine increased the mass of all ceramide acyl chain species, most obviously enhancing the C16 and C18 species ( Fig. 9 A), and as suggested from the labeling experiments ( Fig. 8 B), expression of SphK1 reduced, whereas SphK2 increased all ceramide species ( Fig. 9 A).	transcription
67016	2	336158	5	NULL	NULL	NULL	NULL	sphingosine	Chemical	exogenous	enhances					C16 ceramide	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_44_37118_s_249	16118219	Exogenous sphingosine increased the mass of all ceramide acyl chain species, most obviously enhancing the C16 and C18 species ( Fig. 9 A), and as suggested from the labeling experiments ( Fig. 8 B), expression of SphK1 reduced, whereas SphK2 increased all ceramide species ( Fig. 9 A).	transcription
67017	3	336158	5	NULL	NULL	0	NULL	sphingosine	Chemical	exogenous	enhances					C18 ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_44_37118_s_249	16118219	Exogenous sphingosine increased the mass of all ceramide acyl chain species, most obviously enhancing the C16 and C18 species ( Fig. 9 A), and as suggested from the labeling experiments ( Fig. 8 B), expression of SphK1 reduced, whereas SphK2 increased all ceramide species ( Fig. 9 A).	transcription
67018	4	336158	5	NULL	NULL	NULL	NULL	SphK1	GP	expression of	reduce					ceramide species	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_44_37118_s_249	16118219	Exogenous sphingosine increased the mass of all ceramide acyl chain species, most obviously enhancing the C16 and C18 species ( Fig. 9 A), and as suggested from the labeling experiments ( Fig. 8 B), expression of SphK1 reduced, whereas SphK2 increased all ceramide species ( Fig. 9 A).	transcription
67019	5	336158	5	NULL	NULL	0	NULL	SphK2	GP	expression of	increases					ceramide species	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_44_37118_s_249	16118219	Exogenous sphingosine increased the mass of all ceramide acyl chain species, most obviously enhancing the C16 and C18 species ( Fig. 9 A), and as suggested from the labeling experiments ( Fig. 8 B), expression of SphK1 reduced, whereas SphK2 increased all ceramide species ( Fig. 9 A).	transcription
71184	1	336158	7	NULL	NULL	0	NULL	sphingosine	Chemical	exogenous	increase					ceramide acyl chain species	Chemical	mass of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_44_37118_s_249	16118219	Exogenous sphingosine increased the mass of all ceramide acyl chain species, most obviously enhancing the C16 and C18 species ( Fig. 9 A), and as suggested from the labeling experiments ( Fig. 8 B), expression of SphK1 reduced, whereas SphK2 increased all ceramide species ( Fig. 9 A).	transcription
71185	2	336158	7	NULL	NULL	NULL	NULL	statement 1	Process		enhance					C16 species	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_44_37118_s_249	16118219	Exogenous sphingosine increased the mass of all ceramide acyl chain species, most obviously enhancing the C16 and C18 species ( Fig. 9 A), and as suggested from the labeling experiments ( Fig. 8 B), expression of SphK1 reduced, whereas SphK2 increased all ceramide species ( Fig. 9 A).	transcription
71187	3	336158	7	NULL	NULL	0	NULL	statement 1	Process		enhance					C18 species	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_44_37118_s_249	16118219	Exogenous sphingosine increased the mass of all ceramide acyl chain species, most obviously enhancing the C16 and C18 species ( Fig. 9 A), and as suggested from the labeling experiments ( Fig. 8 B), expression of SphK1 reduced, whereas SphK2 increased all ceramide species ( Fig. 9 A).	transcription
71191	4	336158	7	NULL	NULL	NULL	NULL	SphK1	GP	expression of	reduce					ceramide species	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_44_37118_s_249	16118219	Exogenous sphingosine increased the mass of all ceramide acyl chain species, most obviously enhancing the C16 and C18 species ( Fig. 9 A), and as suggested from the labeling experiments ( Fig. 8 B), expression of SphK1 reduced, whereas SphK2 increased all ceramide species ( Fig. 9 A).	transcription
71193	5	336158	7	NULL	NULL	0	NULL	SphK2	GP		increase					ceramide species	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_44_37118_s_249	16118219	Exogenous sphingosine increased the mass of all ceramide acyl chain species, most obviously enhancing the C16 and C18 species ( Fig. 9 A), and as suggested from the labeling experiments ( Fig. 8 B), expression of SphK1 reduced, whereas SphK2 increased all ceramide species ( Fig. 9 A).	transcription
67020	1	336159	5	NULL	NULL	0	NULL	fumonisin B1	Chemical		inhibits					ceramide	Chemical	formation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_4_2606_s_11	15546881	This conclusion was based on the following: 1) the ability of fumonisin B1 but not myriocin to inhibit ceramide formation, 2) the ability of PMA to induce increases in palmitate-labeled ceramide only under chase labeling but not acute pulse labeling, 3) the induction of the levels of sphingosine but not dihydrosphingosine in response to PMA, and 4) induction of sphingomyelin hydrolysis in response to PMA.	transcription
67021	2	336159	5	NULL	NULL	0	NULL	myriocin	Chemical		does not inhibit					ceramide	Chemical	formation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_4_2606_s_11	15546881	This conclusion was based on the following: 1) the ability of fumonisin B1 but not myriocin to inhibit ceramide formation, 2) the ability of PMA to induce increases in palmitate-labeled ceramide only under chase labeling but not acute pulse labeling, 3) the induction of the levels of sphingosine but not dihydrosphingosine in response to PMA, and 4) induction of sphingomyelin hydrolysis in response to PMA.	transcription
67022	3	336159	5	NULL	NULL	0	NULL	PMA	Chemical		increases					ceramide	Chemical	palmitate-labeled			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_4_2606_s_11	15546881	This conclusion was based on the following: 1) the ability of fumonisin B1 but not myriocin to inhibit ceramide formation, 2) the ability of PMA to induce increases in palmitate-labeled ceramide only under chase labeling but not acute pulse labeling, 3) the induction of the levels of sphingosine but not dihydrosphingosine in response to PMA, and 4) induction of sphingomyelin hydrolysis in response to PMA.	transcription
67023	4	336159	5	NULL	NULL	0	NULL	PMA	Chemical		induce					sphingosine	Chemical	level of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_4_2606_s_11	15546881	This conclusion was based on the following: 1) the ability of fumonisin B1 but not myriocin to inhibit ceramide formation, 2) the ability of PMA to induce increases in palmitate-labeled ceramide only under chase labeling but not acute pulse labeling, 3) the induction of the levels of sphingosine but not dihydrosphingosine in response to PMA, and 4) induction of sphingomyelin hydrolysis in response to PMA.	transcription
67024	5	336159	5	NULL	NULL	0	NULL	PMA	Chemical		does not induce					dihydrosphingosine	Chemical	level of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_4_2606_s_11	15546881	This conclusion was based on the following: 1) the ability of fumonisin B1 but not myriocin to inhibit ceramide formation, 2) the ability of PMA to induce increases in palmitate-labeled ceramide only under chase labeling but not acute pulse labeling, 3) the induction of the levels of sphingosine but not dihydrosphingosine in response to PMA, and 4) induction of sphingomyelin hydrolysis in response to PMA.	transcription
67025	6	336159	5	NULL	NULL	0	NULL	PMA	Chemical		induce					sphingomyelin	Chemical	hydrolysis of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_4_2606_s_11	15546881	This conclusion was based on the following: 1) the ability of fumonisin B1 but not myriocin to inhibit ceramide formation, 2) the ability of PMA to induce increases in palmitate-labeled ceramide only under chase labeling but not acute pulse labeling, 3) the induction of the levels of sphingosine but not dihydrosphingosine in response to PMA, and 4) induction of sphingomyelin hydrolysis in response to PMA.	transcription
71234	1	336159	7	NULL	NULL	0	NULL	fumonisin B1	Chemical		inhibit					ceramide	Chemical	formation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_4_2606_s_11	15546881	This conclusion was based on the following: 1) the ability of fumonisin B1 but not myriocin to inhibit ceramide formation, 2) the ability of PMA to induce increases in palmitate-labeled ceramide only under chase labeling but not acute pulse labeling, 3) the induction of the levels of sphingosine but not dihydrosphingosine in response to PMA, and 4) induction of sphingomyelin hydrolysis in response to PMA.	transcription
71235	2	336159	7	NULL	NULL	0	NULL	myriocin	Chemical		does not inhibit					ceramide	Chemical	formation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_4_2606_s_11	15546881	This conclusion was based on the following: 1) the ability of fumonisin B1 but not myriocin to inhibit ceramide formation, 2) the ability of PMA to induce increases in palmitate-labeled ceramide only under chase labeling but not acute pulse labeling, 3) the induction of the levels of sphingosine but not dihydrosphingosine in response to PMA, and 4) induction of sphingomyelin hydrolysis in response to PMA.	transcription
71236	3	336159	7	NULL	NULL	0	NULL	 PMA	Chemical		induce					ceramide	Chemical	increase in palmitate-labeled			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_4_2606_s_11	15546881	This conclusion was based on the following: 1) the ability of fumonisin B1 but not myriocin to inhibit ceramide formation, 2) the ability of PMA to induce increases in palmitate-labeled ceramide only under chase labeling but not acute pulse labeling, 3) the induction of the levels of sphingosine but not dihydrosphingosine in response to PMA, and 4) induction of sphingomyelin hydrolysis in response to PMA.	transcription
71237	4	336159	7	NULL	NULL	0	NULL	PMA	Chemical		induce					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_4_2606_s_11	15546881	This conclusion was based on the following: 1) the ability of fumonisin B1 but not myriocin to inhibit ceramide formation, 2) the ability of PMA to induce increases in palmitate-labeled ceramide only under chase labeling but not acute pulse labeling, 3) the induction of the levels of sphingosine but not dihydrosphingosine in response to PMA, and 4) induction of sphingomyelin hydrolysis in response to PMA.	transcription
71238	5	336159	7	NULL	NULL	0	NULL	PMA	Chemical		does not induce					dihydrosphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_4_2606_s_11	15546881	This conclusion was based on the following: 1) the ability of fumonisin B1 but not myriocin to inhibit ceramide formation, 2) the ability of PMA to induce increases in palmitate-labeled ceramide only under chase labeling but not acute pulse labeling, 3) the induction of the levels of sphingosine but not dihydrosphingosine in response to PMA, and 4) induction of sphingomyelin hydrolysis in response to PMA.	transcription
71239	6	336159	7	NULL	NULL	0	NULL	PMA	Chemical		induce					sphingomyelin	Chemical	hydrolysis of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_4_2606_s_11	15546881	This conclusion was based on the following: 1) the ability of fumonisin B1 but not myriocin to inhibit ceramide formation, 2) the ability of PMA to induce increases in palmitate-labeled ceramide only under chase labeling but not acute pulse labeling, 3) the induction of the levels of sphingosine but not dihydrosphingosine in response to PMA, and 4) induction of sphingomyelin hydrolysis in response to PMA.	transcription
67026	1	336160	5	NULL	NULL	0	NULL	AC	GP	recombinant	catalyzes					ceramide	Chemical	degradation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_35_32978_s_34	12815059	We find that many properties of the recombinant enzyme are similar to  those reported previously for enzyme obtained from natural sources and that in  addition to ceramide degradation, recombinant AC could catalyze ceramide  synthesis using free fatty acid and sphingosine as substrates.	transcription
67027	2	336160	5	NULL	NULL	0	NULL	AC	GP	recombinant	catalyzes					ceramide	Chemical	synthesis of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_35_32978_s_34	12815059	We find that many properties of the recombinant enzyme are similar to  those reported previously for enzyme obtained from natural sources and that in  addition to ceramide degradation, recombinant AC could catalyze ceramide  synthesis using free fatty acid and sphingosine as substrates.	transcription
67028	3	336160	5	NULL	NULL	0	NULL	fatty acid	Chemical	free	is a substrate for					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_35_32978_s_34	12815059	We find that many properties of the recombinant enzyme are similar to  those reported previously for enzyme obtained from natural sources and that in  addition to ceramide degradation, recombinant AC could catalyze ceramide  synthesis using free fatty acid and sphingosine as substrates.	transcription
67029	4	336160	5	NULL	NULL	0	NULL	sphingosine	Chemical		is a substrate for					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_35_32978_s_34	12815059	We find that many properties of the recombinant enzyme are similar to  those reported previously for enzyme obtained from natural sources and that in  addition to ceramide degradation, recombinant AC could catalyze ceramide  synthesis using free fatty acid and sphingosine as substrates.	transcription
71240	1	336160	7	NULL	NULL	0	NULL	AC 	GP	recombinant	catalyze					 ceramide 	Chemical	synthesis of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_35_32978_s_34	12815059	We find that many properties of the recombinant enzyme are similar to  those reported previously for enzyme obtained from natural sources and that in  addition to ceramide degradation, recombinant AC could catalyze ceramide  synthesis using free fatty acid and sphingosine as substrates.	transcription
71241	2	336160	7	NULL	NULL	0	NULL	sphingosine	Chemical		act as					substrate	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_35_32978_s_34	12815059	We find that many properties of the recombinant enzyme are similar to  those reported previously for enzyme obtained from natural sources and that in  addition to ceramide degradation, recombinant AC could catalyze ceramide  synthesis using free fatty acid and sphingosine as substrates.	transcription
71242	3	336160	7	NULL	NULL	0	NULL	free fatty acid	Chemical		act as					substrate	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_35_32978_s_34	12815059	We find that many properties of the recombinant enzyme are similar to  those reported previously for enzyme obtained from natural sources and that in  addition to ceramide degradation, recombinant AC could catalyze ceramide  synthesis using free fatty acid and sphingosine as substrates.	transcription
71243	4	336160	7	NULL	NULL	0	NULL	statement 2	Process		occur along with					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_35_32978_s_34	12815059	We find that many properties of the recombinant enzyme are similar to  those reported previously for enzyme obtained from natural sources and that in  addition to ceramide degradation, recombinant AC could catalyze ceramide  synthesis using free fatty acid and sphingosine as substrates.	transcription
71244	5	336160	7	NULL	NULL	NULL	NULL	AC	Chemical	recombinant	catalyze					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_35_32978_s_34	12815059	We find that many properties of the recombinant enzyme are similar to  those reported previously for enzyme obtained from natural sources and that in  addition to ceramide degradation, recombinant AC could catalyze ceramide  synthesis using free fatty acid and sphingosine as substrates.	transcription
71245	6	336160	7	NULL	NULL	0	NULL	AC	GP	recombinant	catalyze					ceramide	Chemical	degradation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_35_32978_s_34	12815059	We find that many properties of the recombinant enzyme are similar to  those reported previously for enzyme obtained from natural sources and that in  addition to ceramide degradation, recombinant AC could catalyze ceramide  synthesis using free fatty acid and sphingosine as substrates.	transcription
67030	1	336161	5	NULL	NULL	0	NULL	ceramide	Chemical	synthesis of	is involved in		potentially			PA	Chemical	growth-limiting properties of			NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_1_118_s_192	12518030	To further evaluate if ceramide synthesis could be involved in the growth-limiting properties of PA and TTA, we cultivated PA and TTA-treated D54Mg ( Fig. 7C) and BT4Cn ( Fig. 7D) cells in the absence or presence of sphingosine 1-phosphate, a compound that is known to prevent ceramide-mediated apoptosis ( ), and four different inhibitors of enzymes involved in sphingolipid metabolism.	transcription
67031	2	336161	5	NULL	NULL	0	NULL	ceramide	Chemical	synthesis of	is involved in		potentially			TTA	Chemical	growth-limiting properties of 			NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_1_118_s_192	12518030	To further evaluate if ceramide synthesis could be involved in the growth-limiting properties of PA and TTA, we cultivated PA and TTA-treated D54Mg ( Fig. 7C) and BT4Cn ( Fig. 7D) cells in the absence or presence of sphingosine 1-phosphate, a compound that is known to prevent ceramide-mediated apoptosis ( ), and four different inhibitors of enzymes involved in sphingolipid metabolism.	transcription
67032	3	336161	5	NULL	NULL	0	NULL	apoptosis	Process		is mediated by					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_1_118_s_192	12518030	To further evaluate if ceramide synthesis could be involved in the growth-limiting properties of PA and TTA, we cultivated PA and TTA-treated D54Mg ( Fig. 7C) and BT4Cn ( Fig. 7D) cells in the absence or presence of sphingosine 1-phosphate, a compound that is known to prevent ceramide-mediated apoptosis ( ), and four different inhibitors of enzymes involved in sphingolipid metabolism.	transcription
67033	4	336161	5	NULL	NULL	0	NULL	sphingosine 1-phosphate	Chemical		prevents					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_1_118_s_192	12518030	To further evaluate if ceramide synthesis could be involved in the growth-limiting properties of PA and TTA, we cultivated PA and TTA-treated D54Mg ( Fig. 7C) and BT4Cn ( Fig. 7D) cells in the absence or presence of sphingosine 1-phosphate, a compound that is known to prevent ceramide-mediated apoptosis ( ), and four different inhibitors of enzymes involved in sphingolipid metabolism.	transcription
71272	1	336161	7	NULL	NULL	0	NULL	ceramide	Chemical		mediates					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_1_118_s_192	12518030	To further evaluate if ceramide synthesis could be involved in the growth-limiting properties of PA and TTA, we cultivated PA and TTA-treated D54Mg ( Fig. 7C) and BT4Cn ( Fig. 7D) cells in the absence or presence of sphingosine 1-phosphate, a compound that is known to prevent ceramide-mediated apoptosis ( ), and four different inhibitors of enzymes involved in sphingolipid metabolism.	transcription
71273	2	336161	7	NULL	NULL	0	NULL	sphingosine 1-phosphate	Chemical		prevent					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_1_118_s_192	12518030	To further evaluate if ceramide synthesis could be involved in the growth-limiting properties of PA and TTA, we cultivated PA and TTA-treated D54Mg ( Fig. 7C) and BT4Cn ( Fig. 7D) cells in the absence or presence of sphingosine 1-phosphate, a compound that is known to prevent ceramide-mediated apoptosis ( ), and four different inhibitors of enzymes involved in sphingolipid metabolism.	transcription
67034	1	336162	5	NULL	NULL	0	NULL	ceramide	Chemical	M. sexta	induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw70_jlipidres_45_7_1221_s_245	15102888	The results provided initial evidence suggesting that the ceramide mixture obtained from stage 12  M. sexta is more effective in inducing apoptosis than the commercial ceramide lacking extra unsaturation, supporting the hypothesis that the extra unsaturation at C-6 of the sphingosine enhances apoptosis.	transcription
67035	2	336162	5	NULL	NULL	0	NULL	ceramide	Chemical	commercial	induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw70_jlipidres_45_7_1221_s_245	15102888	The results provided initial evidence suggesting that the ceramide mixture obtained from stage 12  M. sexta is more effective in inducing apoptosis than the commercial ceramide lacking extra unsaturation, supporting the hypothesis that the extra unsaturation at C-6 of the sphingosine enhances apoptosis.	transcription
67036	3	336162	5	NULL	NULL	0	NULL	statement 1	Process		more effective than					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_jlipidres_45_7_1221_s_245	15102888	The results provided initial evidence suggesting that the ceramide mixture obtained from stage 12  M. sexta is more effective in inducing apoptosis than the commercial ceramide lacking extra unsaturation, supporting the hypothesis that the extra unsaturation at C-6 of the sphingosine enhances apoptosis.	transcription
67037	4	336162	5	NULL	NULL	0	NULL	sphingosine	Chemical	extra unsaturation at C-6 of	enhances					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw70_jlipidres_45_7_1221_s_245	15102888	The results provided initial evidence suggesting that the ceramide mixture obtained from stage 12  M. sexta is more effective in inducing apoptosis than the commercial ceramide lacking extra unsaturation, supporting the hypothesis that the extra unsaturation at C-6 of the sphingosine enhances apoptosis.	transcription
67038	5	336162	5	NULL	NULL	0	NULL	ceramide	Chemical	commercial	lacks					unsaturation	Process	extra			NULL		0	NULL	NULL	NULL	gw70_jlipidres_45_7_1221_s_245	15102888	The results provided initial evidence suggesting that the ceramide mixture obtained from stage 12  M. sexta is more effective in inducing apoptosis than the commercial ceramide lacking extra unsaturation, supporting the hypothesis that the extra unsaturation at C-6 of the sphingosine enhances apoptosis.	transcription
71274	1	336162	7	NULL	NULL	0	NULL	ceramide mixture	Chemical		obtained from					stage 12 M. sexta	Organism				NULL		0	NULL	NULL	NULL	gw70_jlipidres_45_7_1221_s_245	15102888	The results provided initial evidence suggesting that the ceramide mixture obtained from stage 12  M. sexta is more effective in inducing apoptosis than the commercial ceramide lacking extra unsaturation, supporting the hypothesis that the extra unsaturation at C-6 of the sphingosine enhances apoptosis.	transcription
71275	2	336162	7	NULL	NULL	0	NULL	statement 1	Process		induce		effectively			apoptosis	Process				NULL		0	NULL	NULL	NULL	gw70_jlipidres_45_7_1221_s_245	15102888	The results provided initial evidence suggesting that the ceramide mixture obtained from stage 12  M. sexta is more effective in inducing apoptosis than the commercial ceramide lacking extra unsaturation, supporting the hypothesis that the extra unsaturation at C-6 of the sphingosine enhances apoptosis.	transcription
71276	3	336162	7	NULL	NULL	NULL	NULL	sphingosine	Chemical	unsaturation at C-6	enhance					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_45_7_1221_s_245	15102888	The results provided initial evidence suggesting that the ceramide mixture obtained from stage 12  M. sexta is more effective in inducing apoptosis than the commercial ceramide lacking extra unsaturation, supporting the hypothesis that the extra unsaturation at C-6 of the sphingosine enhances apoptosis.	transcription
67039	1	336163	5	NULL	NULL	0	NULL	TID-ceramide	Chemical	radiolabelled	bind					CTSD	GP				NULL		0	NULL	NULL	NULL	gw60_embo_18_19_5252_s_73	10508159	As shown in Figure  2A, D- erythro-C6-ceramide and D- erythro-sphingosine dose-dependently competed for binding of the radiolabeled [125]TID-ceramide, whereas the biologically inactive D- erythro-dihydroceramide and D- erythro-dihydrosphingosine were significantly less potent in competing for TID-ceramide binding to CTSD.	transcription
67040	2	336163	5	NULL	NULL	0	NULL	D- erythro-C6-ceramide	Chemical		bind					CTSD	GP				NULL		0	NULL	NULL	NULL	gw60_embo_18_19_5252_s_73	10508159	As shown in Figure  2A, D- erythro-C6-ceramide and D- erythro-sphingosine dose-dependently competed for binding of the radiolabeled [125]TID-ceramide, whereas the biologically inactive D- erythro-dihydroceramide and D- erythro-dihydrosphingosine were significantly less potent in competing for TID-ceramide binding to CTSD.	transcription
67041	3	336163	5	NULL	NULL	0	NULL	D- erythro-sphingosine	Chemical		bind					CTSD	GP				NULL		0	NULL	NULL	NULL	gw60_embo_18_19_5252_s_73	10508159	As shown in Figure  2A, D- erythro-C6-ceramide and D- erythro-sphingosine dose-dependently competed for binding of the radiolabeled [125]TID-ceramide, whereas the biologically inactive D- erythro-dihydroceramide and D- erythro-dihydrosphingosine were significantly less potent in competing for TID-ceramide binding to CTSD.	transcription
67042	4	336163	5	NULL	NULL	0	NULL	statement 2	Process		competes with		dose dependently			statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_19_5252_s_73	10508159	As shown in Figure  2A, D- erythro-C6-ceramide and D- erythro-sphingosine dose-dependently competed for binding of the radiolabeled [125]TID-ceramide, whereas the biologically inactive D- erythro-dihydroceramide and D- erythro-dihydrosphingosine were significantly less potent in competing for TID-ceramide binding to CTSD.	transcription
67043	5	336163	5	NULL	NULL	0	NULL	statement 3	Process		competes with		dose dependently			statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_19_5252_s_73	10508159	As shown in Figure  2A, D- erythro-C6-ceramide and D- erythro-sphingosine dose-dependently competed for binding of the radiolabeled [125]TID-ceramide, whereas the biologically inactive D- erythro-dihydroceramide and D- erythro-dihydrosphingosine were significantly less potent in competing for TID-ceramide binding to CTSD.	transcription
67044	6	336163	5	NULL	NULL	0	NULL	D- erythro-dihydroceramide	Chemical	biologically inactive	bind					CTSD	GP				NULL		0	NULL	NULL	NULL	gw60_embo_18_19_5252_s_73	10508159	As shown in Figure  2A, D- erythro-C6-ceramide and D- erythro-sphingosine dose-dependently competed for binding of the radiolabeled [125]TID-ceramide, whereas the biologically inactive D- erythro-dihydroceramide and D- erythro-dihydrosphingosine were significantly less potent in competing for TID-ceramide binding to CTSD.	transcription
67045	7	336163	5	NULL	NULL	0	NULL	D- erythro-dihydrosphingosine	Chemical		bind					CTSD	GP				NULL		0	NULL	NULL	NULL	gw60_embo_18_19_5252_s_73	10508159	As shown in Figure  2A, D- erythro-C6-ceramide and D- erythro-sphingosine dose-dependently competed for binding of the radiolabeled [125]TID-ceramide, whereas the biologically inactive D- erythro-dihydroceramide and D- erythro-dihydrosphingosine were significantly less potent in competing for TID-ceramide binding to CTSD.	transcription
67046	8	336163	5	NULL	NULL	NULL	NULL	statement 7	Process		competes with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_19_5252_s_73	10508159	As shown in Figure  2A, D- erythro-C6-ceramide and D- erythro-sphingosine dose-dependently competed for binding of the radiolabeled [125]TID-ceramide, whereas the biologically inactive D- erythro-dihydroceramide and D- erythro-dihydrosphingosine were significantly less potent in competing for TID-ceramide binding to CTSD.	transcription
67047	9	336163	5	NULL	NULL	NULL	NULL	statement 6	Process		competes with					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_19_5252_s_73	10508159	As shown in Figure  2A, D- erythro-C6-ceramide and D- erythro-sphingosine dose-dependently competed for binding of the radiolabeled [125]TID-ceramide, whereas the biologically inactive D- erythro-dihydroceramide and D- erythro-dihydrosphingosine were significantly less potent in competing for TID-ceramide binding to CTSD.	transcription
67048	10	336163	5	NULL	NULL	0	NULL	statement 8	Process		less potent than					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_19_5252_s_73	10508159	As shown in Figure  2A, D- erythro-C6-ceramide and D- erythro-sphingosine dose-dependently competed for binding of the radiolabeled [125]TID-ceramide, whereas the biologically inactive D- erythro-dihydroceramide and D- erythro-dihydrosphingosine were significantly less potent in competing for TID-ceramide binding to CTSD.	transcription
67049	11	336163	5	NULL	NULL	NULL	NULL	statement 8	Process		less potent than					statement 5	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_19_5252_s_73	10508159	As shown in Figure  2A, D- erythro-C6-ceramide and D- erythro-sphingosine dose-dependently competed for binding of the radiolabeled [125]TID-ceramide, whereas the biologically inactive D- erythro-dihydroceramide and D- erythro-dihydrosphingosine were significantly less potent in competing for TID-ceramide binding to CTSD.	transcription
67050	12	336163	5	NULL	NULL	0	NULL	statement 9	Process		less potent than					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_19_5252_s_73	10508159	As shown in Figure  2A, D- erythro-C6-ceramide and D- erythro-sphingosine dose-dependently competed for binding of the radiolabeled [125]TID-ceramide, whereas the biologically inactive D- erythro-dihydroceramide and D- erythro-dihydrosphingosine were significantly less potent in competing for TID-ceramide binding to CTSD.	transcription
67051	13	336163	5	NULL	NULL	0	NULL	statement 9	Process		less potent than					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_embo_18_19_5252_s_73	10508159	As shown in Figure  2A, D- erythro-C6-ceramide and D- erythro-sphingosine dose-dependently competed for binding of the radiolabeled [125]TID-ceramide, whereas the biologically inactive D- erythro-dihydroceramide and D- erythro-dihydrosphingosine were significantly less potent in competing for TID-ceramide binding to CTSD.	transcription
71277	2	336163	7	NULL	NULL	NULL	NULL	D- erythro-C6-ceramide	Chemical		compete with		dose-dependently			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_19_5252_s_73	10508159	As shown in Figure  2A, D- erythro-C6-ceramide and D- erythro-sphingosine dose-dependently competed for binding of the radiolabeled [125]TID-ceramide, whereas the biologically inactive D- erythro-dihydroceramide and D- erythro-dihydrosphingosine were significantly less potent in competing for TID-ceramide binding to CTSD.	transcription
71278	2	336163	7	NULL	NULL	NULL	NULL	D- erythro-sphingosine	Chemical		compete with		dose-dependently			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_19_5252_s_73	10508159	As shown in Figure  2A, D- erythro-C6-ceramide and D- erythro-sphingosine dose-dependently competed for binding of the radiolabeled [125]TID-ceramide, whereas the biologically inactive D- erythro-dihydroceramide and D- erythro-dihydrosphingosine were significantly less potent in competing for TID-ceramide binding to CTSD.	transcription
71279	1	336163	7	NULL	NULL	NULL	NULL	[125]TID-ceramide	Chemical	radiolabeled	bind					CTSD	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_19_5252_s_73	10508159	As shown in Figure  2A, D- erythro-C6-ceramide and D- erythro-sphingosine dose-dependently competed for binding of the radiolabeled [125]TID-ceramide, whereas the biologically inactive D- erythro-dihydroceramide and D- erythro-dihydrosphingosine were significantly less potent in competing for TID-ceramide binding to CTSD.	transcription
71280	4	336163	7	NULL	NULL	0	NULL	TID-ceramide	Chemical		bind					CTSD	Chemical				NULL		0	NULL	NULL	NULL	gw60_embo_18_19_5252_s_73	10508159	As shown in Figure  2A, D- erythro-C6-ceramide and D- erythro-sphingosine dose-dependently competed for binding of the radiolabeled [125]TID-ceramide, whereas the biologically inactive D- erythro-dihydroceramide and D- erythro-dihydrosphingosine were significantly less potent in competing for TID-ceramide binding to CTSD.	transcription
71281	5	336163	7	NULL	NULL	NULL	NULL	D- erythro-dihydroceramide	Chemical	biologically inactive	compete with		less potently			statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_19_5252_s_73	10508159	As shown in Figure  2A, D- erythro-C6-ceramide and D- erythro-sphingosine dose-dependently competed for binding of the radiolabeled [125]TID-ceramide, whereas the biologically inactive D- erythro-dihydroceramide and D- erythro-dihydrosphingosine were significantly less potent in competing for TID-ceramide binding to CTSD.	transcription
71282	6	336163	7	NULL	NULL	NULL	NULL	D- erythro-dihydrosphingosine	Chemical	biologically inactive	compete with		less potently			statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_embo_18_19_5252_s_73	10508159	As shown in Figure  2A, D- erythro-C6-ceramide and D- erythro-sphingosine dose-dependently competed for binding of the radiolabeled [125]TID-ceramide, whereas the biologically inactive D- erythro-dihydroceramide and D- erythro-dihydrosphingosine were significantly less potent in competing for TID-ceramide binding to CTSD.	transcription
67052	1	336164	5	NULL	NULL	0	NULL	ceramide	Chemical	elevation of;;plasma	is induced by					LPS	Chemical				NULL		0	NULL	NULL	NULL	gw60_brainres_895_1_59_s_166	11259760	Evidence from experiments on macrophage cell lines, which have been shown to produce ceramide in response to LPS [ 23], and on human neutrophils, which upregulate sphingosine levels in response to various agonists [  47], suggests that blood cells could also contribute to LPS-induced plasma ceramide elevation.	transcription
67053	2	336164	5	NULL	NULL	0	NULL	blood cells	Cell		contribute to					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_brainres_895_1_59_s_166	11259760	Evidence from experiments on macrophage cell lines, which have been shown to produce ceramide in response to LPS [ 23], and on human neutrophils, which upregulate sphingosine levels in response to various agonists [  47], suggests that blood cells could also contribute to LPS-induced plasma ceramide elevation.	transcription
67054	3	336164	5	NULL	NULL	NULL	NULL	ceramide	Chemical		is produced					LPS	Chemical	in response to			NULL	macrophage cell lines	NULL	NULL	NULL	NULL	gw60_brainres_895_1_59_s_166	11259760	Evidence from experiments on macrophage cell lines, which have been shown to produce ceramide in response to LPS [ 23], and on human neutrophils, which upregulate sphingosine levels in response to various agonists [  47], suggests that blood cells could also contribute to LPS-induced plasma ceramide elevation.	transcription
67055	4	336164	5	NULL	NULL	0	NULL	agonists	Chemical		upregulates					sphingosine	Chemical	levels of			NULL	human neutrophils	0	NULL	NULL	NULL	gw60_brainres_895_1_59_s_166	11259760	Evidence from experiments on macrophage cell lines, which have been shown to produce ceramide in response to LPS [ 23], and on human neutrophils, which upregulate sphingosine levels in response to various agonists [  47], suggests that blood cells could also contribute to LPS-induced plasma ceramide elevation.	transcription
71283	1	336164	7	NULL	NULL	0	NULL	LPS	Chemical		produce					ceramide	Chemical				NULL	macrophage cell lines	0	NULL	NULL	NULL	gw60_brainres_895_1_59_s_166	11259760	Evidence from experiments on macrophage cell lines, which have been shown to produce ceramide in response to LPS [ 23], and on human neutrophils, which upregulate sphingosine levels in response to various agonists [  47], suggests that blood cells could also contribute to LPS-induced plasma ceramide elevation.	transcription
71284	2	336164	7	NULL	NULL	0	NULL	LPS	Chemical		induce					plasma ceramide	Chemical	elevation of			NULL		0	NULL	NULL	NULL	gw60_brainres_895_1_59_s_166	11259760	Evidence from experiments on macrophage cell lines, which have been shown to produce ceramide in response to LPS [ 23], and on human neutrophils, which upregulate sphingosine levels in response to various agonists [  47], suggests that blood cells could also contribute to LPS-induced plasma ceramide elevation.	transcription
71285	3	336164	7	NULL	NULL	0	NULL	blood cells	Cell		contribute to					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_brainres_895_1_59_s_166	11259760	Evidence from experiments on macrophage cell lines, which have been shown to produce ceramide in response to LPS [ 23], and on human neutrophils, which upregulate sphingosine levels in response to various agonists [  47], suggests that blood cells could also contribute to LPS-induced plasma ceramide elevation.	transcription
67060	1	336165	5	NULL	NULL	0	NULL	apoptosis	Process		is induced by					serum deprivation	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_302	10545499	Our present results show that expression of sphingosine kinase in 3T3 fibroblasts, HEK 293, and Jurkat T cells suppressed apoptosis induced by serum deprivation, known to increase ceramide levels, or by the ceramide analogue, C2-ceramide, with concomitant inhibition of activation of the executionary caspase-3.	transcription
67061	2	336165	5	NULL	NULL	0	NULL	sphingosine kinase	GP		is expressed in					3T3 fibroblasts	Cell				NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_302	10545499	Our present results show that expression of sphingosine kinase in 3T3 fibroblasts, HEK 293, and Jurkat T cells suppressed apoptosis induced by serum deprivation, known to increase ceramide levels, or by the ceramide analogue, C2-ceramide, with concomitant inhibition of activation of the executionary caspase-3.	transcription
67062	3	336165	5	NULL	NULL	0	NULL	sphingosine kinase	GP		is expressed in					HEK 293	Cell				NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_302	10545499	Our present results show that expression of sphingosine kinase in 3T3 fibroblasts, HEK 293, and Jurkat T cells suppressed apoptosis induced by serum deprivation, known to increase ceramide levels, or by the ceramide analogue, C2-ceramide, with concomitant inhibition of activation of the executionary caspase-3.	transcription
67063	4	336165	5	NULL	NULL	0	NULL	sphingosine kinase	GP		is expressed in					Jurkat T cells	Cell				NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_302	10545499	Our present results show that expression of sphingosine kinase in 3T3 fibroblasts, HEK 293, and Jurkat T cells suppressed apoptosis induced by serum deprivation, known to increase ceramide levels, or by the ceramide analogue, C2-ceramide, with concomitant inhibition of activation of the executionary caspase-3.	transcription
67064	5	336165	5	NULL	NULL	0	NULL	statement 2	Process		suppress					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_302	10545499	Our present results show that expression of sphingosine kinase in 3T3 fibroblasts, HEK 293, and Jurkat T cells suppressed apoptosis induced by serum deprivation, known to increase ceramide levels, or by the ceramide analogue, C2-ceramide, with concomitant inhibition of activation of the executionary caspase-3.	transcription
67065	6	336165	5	NULL	NULL	0	NULL	statement 3	Process		suppress					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_302	10545499	Our present results show that expression of sphingosine kinase in 3T3 fibroblasts, HEK 293, and Jurkat T cells suppressed apoptosis induced by serum deprivation, known to increase ceramide levels, or by the ceramide analogue, C2-ceramide, with concomitant inhibition of activation of the executionary caspase-3.	transcription
67066	7	336165	5	NULL	NULL	0	NULL	statement 4	Process		suppress					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_302	10545499	Our present results show that expression of sphingosine kinase in 3T3 fibroblasts, HEK 293, and Jurkat T cells suppressed apoptosis induced by serum deprivation, known to increase ceramide levels, or by the ceramide analogue, C2-ceramide, with concomitant inhibition of activation of the executionary caspase-3.	transcription
67067	8	336165	5	NULL	NULL	0	NULL	statement 1	Process		increases					ceramide	Chemical	level of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_302	10545499	Our present results show that expression of sphingosine kinase in 3T3 fibroblasts, HEK 293, and Jurkat T cells suppressed apoptosis induced by serum deprivation, known to increase ceramide levels, or by the ceramide analogue, C2-ceramide, with concomitant inhibition of activation of the executionary caspase-3.	transcription
67068	9	336165	5	NULL	NULL	NULL	NULL	C2-ceramide	Chemical		is an analogue of					ceramide	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_302	10545499	Our present results show that expression of sphingosine kinase in 3T3 fibroblasts, HEK 293, and Jurkat T cells suppressed apoptosis induced by serum deprivation, known to increase ceramide levels, or by the ceramide analogue, C2-ceramide, with concomitant inhibition of activation of the executionary caspase-3.	transcription
71286	1	336165	7	NULL	NULL	0	NULL	serum 	OrganismPart	deprivation of	induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_302	10545499	Our present results show that expression of sphingosine kinase in 3T3 fibroblasts, HEK 293, and Jurkat T cells suppressed apoptosis induced by serum deprivation, known to increase ceramide levels, or by the ceramide analogue, C2-ceramide, with concomitant inhibition of activation of the executionary caspase-3.	transcription
71287	2	336165	7	NULL	NULL	0	NULL	sphingosine kinase	GP		suppress					statement 1	Process				NULL	3T3 fibroblasts	0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_302	10545499	Our present results show that expression of sphingosine kinase in 3T3 fibroblasts, HEK 293, and Jurkat T cells suppressed apoptosis induced by serum deprivation, known to increase ceramide levels, or by the ceramide analogue, C2-ceramide, with concomitant inhibition of activation of the executionary caspase-3.	transcription
71288	3	336165	7	NULL	NULL	NULL	NULL	sphingosine kinase	GP		suppress					statement 1	Process				NULL	HEK 293 cells	NULL	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_302	10545499	Our present results show that expression of sphingosine kinase in 3T3 fibroblasts, HEK 293, and Jurkat T cells suppressed apoptosis induced by serum deprivation, known to increase ceramide levels, or by the ceramide analogue, C2-ceramide, with concomitant inhibition of activation of the executionary caspase-3.	transcription
71289	4	336165	7	NULL	NULL	NULL	NULL	sphingosine kinase	GP		suppress					statement 1	Process				NULL	Jurkat T cells	NULL	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_302	10545499	Our present results show that expression of sphingosine kinase in 3T3 fibroblasts, HEK 293, and Jurkat T cells suppressed apoptosis induced by serum deprivation, known to increase ceramide levels, or by the ceramide analogue, C2-ceramide, with concomitant inhibition of activation of the executionary caspase-3.	transcription
71290	5	336165	7	NULL	NULL	0	NULL	sphingosine kinase	GP		increase					ceramide	Chemical				NULL	3T3 fibroblasts	0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_302	10545499	Our present results show that expression of sphingosine kinase in 3T3 fibroblasts, HEK 293, and Jurkat T cells suppressed apoptosis induced by serum deprivation, known to increase ceramide levels, or by the ceramide analogue, C2-ceramide, with concomitant inhibition of activation of the executionary caspase-3.	transcription
71291	6	336165	7	NULL	NULL	0	NULL	sphingosine kinase	GP		increase					ceramide	Chemical				NULL	HEK 293 cells	0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_302	10545499	Our present results show that expression of sphingosine kinase in 3T3 fibroblasts, HEK 293, and Jurkat T cells suppressed apoptosis induced by serum deprivation, known to increase ceramide levels, or by the ceramide analogue, C2-ceramide, with concomitant inhibition of activation of the executionary caspase-3.	transcription
71292	7	336165	7	NULL	NULL	0	NULL	sphingosine kinase	GP		increase					ceramide	Chemical				NULL	Jurkat T cells	0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_302	10545499	Our present results show that expression of sphingosine kinase in 3T3 fibroblasts, HEK 293, and Jurkat T cells suppressed apoptosis induced by serum deprivation, known to increase ceramide levels, or by the ceramide analogue, C2-ceramide, with concomitant inhibition of activation of the executionary caspase-3.	transcription
71293	8	336165	7	NULL	NULL	0	NULL	sphingosine kinase	GP		increase					C2-ceramide	Chemical				NULL	3T3 fibroblasts	0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_302	10545499	Our present results show that expression of sphingosine kinase in 3T3 fibroblasts, HEK 293, and Jurkat T cells suppressed apoptosis induced by serum deprivation, known to increase ceramide levels, or by the ceramide analogue, C2-ceramide, with concomitant inhibition of activation of the executionary caspase-3.	transcription
71294	9	336165	7	NULL	NULL	0	NULL	sphingosine kinase	GP		increase					C2-ceramide	Chemical				NULL	HEK293 cells	0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_302	10545499	Our present results show that expression of sphingosine kinase in 3T3 fibroblasts, HEK 293, and Jurkat T cells suppressed apoptosis induced by serum deprivation, known to increase ceramide levels, or by the ceramide analogue, C2-ceramide, with concomitant inhibition of activation of the executionary caspase-3.	transcription
71295	10	336165	7	NULL	NULL	0	NULL	sphingosine kinase	GP		increase					C2-ceramide	Chemical				NULL	Jurkat T cells	0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_302	10545499	Our present results show that expression of sphingosine kinase in 3T3 fibroblasts, HEK 293, and Jurkat T cells suppressed apoptosis induced by serum deprivation, known to increase ceramide levels, or by the ceramide analogue, C2-ceramide, with concomitant inhibition of activation of the executionary caspase-3.	transcription
71296	11	336165	7	NULL	NULL	NULL	NULL	sphingosine kinase	GP		inhibit					caspase-3	GP	activation of executionary			NULL	3T3 fibroblasts	NULL	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_302	10545499	Our present results show that expression of sphingosine kinase in 3T3 fibroblasts, HEK 293, and Jurkat T cells suppressed apoptosis induced by serum deprivation, known to increase ceramide levels, or by the ceramide analogue, C2-ceramide, with concomitant inhibition of activation of the executionary caspase-3.	transcription
71297	12	336165	7	NULL	NULL	0	NULL	sphingosine kinase	GP		inhibit					caspase-3	GP	activation of executionary			NULL	HEK293 cells	0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_302	10545499	Our present results show that expression of sphingosine kinase in 3T3 fibroblasts, HEK 293, and Jurkat T cells suppressed apoptosis induced by serum deprivation, known to increase ceramide levels, or by the ceramide analogue, C2-ceramide, with concomitant inhibition of activation of the executionary caspase-3.	transcription
71298	13	336165	7	NULL	NULL	NULL	NULL	sphingosine kinase	GP		inhibit					caspase-3	GP	activation of executionary			NULL	Jurkat T cells	NULL	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_302	10545499	Our present results show that expression of sphingosine kinase in 3T3 fibroblasts, HEK 293, and Jurkat T cells suppressed apoptosis induced by serum deprivation, known to increase ceramide levels, or by the ceramide analogue, C2-ceramide, with concomitant inhibition of activation of the executionary caspase-3.	transcription
71299	14	336165	7	NULL	NULL	0	NULL	C2-ceramide	Chemical		is a type of					ceramide analogue	Chemical				NULL		0	NULL	NULL	NULL	gw60_cellbiol_147_3_545_s_302	10545499	Our present results show that expression of sphingosine kinase in 3T3 fibroblasts, HEK 293, and Jurkat T cells suppressed apoptosis induced by serum deprivation, known to increase ceramide levels, or by the ceramide analogue, C2-ceramide, with concomitant inhibition of activation of the executionary caspase-3.	transcription
67069	1	336166	5	NULL	NULL	0	NULL	sphingosine	Chemical		is a metabolite of					sphingolipid	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13275_s_109	10788433	This appears to be a specific ceramide effect because other related sphingolipid metabolites, including sphingosine and the inactive ceramide analogue, C2-dihydroceramide, which has the same structure as C2-ceramide but lacks the double bond, did not replicate the effects of C2-ceramide or SMase (data not shown).	transcription
67070	2	336166	5	NULL	NULL	0	NULL	C2-dihydroceramide	Chemical		is an analogue of					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13275_s_109	10788433	This appears to be a specific ceramide effect because other related sphingolipid metabolites, including sphingosine and the inactive ceramide analogue, C2-dihydroceramide, which has the same structure as C2-ceramide but lacks the double bond, did not replicate the effects of C2-ceramide or SMase (data not shown).	transcription
67071	3	336166	5	NULL	NULL	0	NULL	C2-dihydroceramide	Chemical		is a metabolite of					sphingolipid	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13275_s_109	10788433	This appears to be a specific ceramide effect because other related sphingolipid metabolites, including sphingosine and the inactive ceramide analogue, C2-dihydroceramide, which has the same structure as C2-ceramide but lacks the double bond, did not replicate the effects of C2-ceramide or SMase (data not shown).	transcription
67072	4	336166	5	NULL	NULL	0	NULL	C2-dihydroceramide	Chemical	structure of	same as					C2-ceramide	Chemical	structure of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13275_s_109	10788433	This appears to be a specific ceramide effect because other related sphingolipid metabolites, including sphingosine and the inactive ceramide analogue, C2-dihydroceramide, which has the same structure as C2-ceramide but lacks the double bond, did not replicate the effects of C2-ceramide or SMase (data not shown).	transcription
67073	5	336166	5	NULL	NULL	NULL	NULL	C2-dihydroceramide	Chemical	inactive	does not replicate					C2-ceramide	Chemical	effects of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_18_13275_s_109	10788433	This appears to be a specific ceramide effect because other related sphingolipid metabolites, including sphingosine and the inactive ceramide analogue, C2-dihydroceramide, which has the same structure as C2-ceramide but lacks the double bond, did not replicate the effects of C2-ceramide or SMase (data not shown).	transcription
67074	6	336166	5	NULL	NULL	0	NULL	C2-dihydroceramide	Chemical	inactive	does not replicate					SMase	GP	effects of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13275_s_109	10788433	This appears to be a specific ceramide effect because other related sphingolipid metabolites, including sphingosine and the inactive ceramide analogue, C2-dihydroceramide, which has the same structure as C2-ceramide but lacks the double bond, did not replicate the effects of C2-ceramide or SMase (data not shown).	transcription
71300	1	336166	7	NULL	NULL	0	NULL	sphingosine	Chemical		is a type of					sphingolipid metabolite	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13275_s_109	10788433	This appears to be a specific ceramide effect because other related sphingolipid metabolites, including sphingosine and the inactive ceramide analogue, C2-dihydroceramide, which has the same structure as C2-ceramide but lacks the double bond, did not replicate the effects of C2-ceramide or SMase (data not shown).	transcription
71301	2	336166	7	NULL	NULL	0	NULL	C2-dihydroceramide	Chemical		is a type of					ceramide analogue	Chemical	inactive			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13275_s_109	10788433	This appears to be a specific ceramide effect because other related sphingolipid metabolites, including sphingosine and the inactive ceramide analogue, C2-dihydroceramide, which has the same structure as C2-ceramide but lacks the double bond, did not replicate the effects of C2-ceramide or SMase (data not shown).	transcription
71302	3	336166	7	NULL	NULL	0	NULL	C2-dihydroceramide	Chemical		lacks					C2-ceramide	Chemical	double bond of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13275_s_109	10788433	This appears to be a specific ceramide effect because other related sphingolipid metabolites, including sphingosine and the inactive ceramide analogue, C2-dihydroceramide, which has the same structure as C2-ceramide but lacks the double bond, did not replicate the effects of C2-ceramide or SMase (data not shown).	transcription
71303	4	336166	7	NULL	NULL	0	NULL	C2-dihydroceramide	Chemical		does not replicate					C2-ceramide	Chemical	effects of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_18_13275_s_109	10788433	This appears to be a specific ceramide effect because other related sphingolipid metabolites, including sphingosine and the inactive ceramide analogue, C2-dihydroceramide, which has the same structure as C2-ceramide but lacks the double bond, did not replicate the effects of C2-ceramide or SMase (data not shown).	transcription
71304	5	336166	7	NULL	NULL	NULL	NULL	C2-dihydroceramide	Chemical		does not replicate					SMase	GP	effects of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_18_13275_s_109	10788433	This appears to be a specific ceramide effect because other related sphingolipid metabolites, including sphingosine and the inactive ceramide analogue, C2-dihydroceramide, which has the same structure as C2-ceramide but lacks the double bond, did not replicate the effects of C2-ceramide or SMase (data not shown).	transcription
67075	1	336167	5	NULL	NULL	0	NULL	apoptosis	Process		is induced by					Fas	GP				NULL	Type II Cells	0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_240	10747891	Potential Involvement of Ceramide and Sphingosine in Fas-induced Apoptosis of Type II Cells-- Abundant reports have suggested that ceramide may play a role in apoptotic signals initiated through the Fas system in various types of cells ( 10- 21, 27, 72).	transcription
67076	2	336167	5	NULL	NULL	0	NULL	ceramide	Chemical		is involved in		potentially			statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_240	10747891	Potential Involvement of Ceramide and Sphingosine in Fas-induced Apoptosis of Type II Cells-- Abundant reports have suggested that ceramide may play a role in apoptotic signals initiated through the Fas system in various types of cells ( 10- 21, 27, 72).	transcription
67077	3	336167	5	NULL	NULL	0	NULL	sphingosine	Chemical		is involved in		potentially			statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_240	10747891	Potential Involvement of Ceramide and Sphingosine in Fas-induced Apoptosis of Type II Cells-- Abundant reports have suggested that ceramide may play a role in apoptotic signals initiated through the Fas system in various types of cells ( 10- 21, 27, 72).	transcription
67078	4	336167	5	NULL	NULL	NULL	NULL	apoptotic signals	Process		initiated through					Fas system	GP				NULL	various types of cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_240	10747891	Potential Involvement of Ceramide and Sphingosine in Fas-induced Apoptosis of Type II Cells-- Abundant reports have suggested that ceramide may play a role in apoptotic signals initiated through the Fas system in various types of cells ( 10- 21, 27, 72).	transcription
67079	5	336167	5	NULL	NULL	0	NULL	ceramide	Chemical		plays a role in		may			statement 4	Process				NULL	various types of cells	0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_240	10747891	Potential Involvement of Ceramide and Sphingosine in Fas-induced Apoptosis of Type II Cells-- Abundant reports have suggested that ceramide may play a role in apoptotic signals initiated through the Fas system in various types of cells ( 10- 21, 27, 72).	transcription
71305	1	336167	7	NULL	NULL	0	NULL	Fas	GP		induce					apoptosis	Process				NULL	Type II cells	0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_240	10747891	Potential Involvement of Ceramide and Sphingosine in Fas-induced Apoptosis of Type II Cells-- Abundant reports have suggested that ceramide may play a role in apoptotic signals initiated through the Fas system in various types of cells ( 10- 21, 27, 72).	transcription
71306	2	336167	7	NULL	NULL	0	NULL	Ceramide	Chemical		play a role in		may			statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_240	10747891	Potential Involvement of Ceramide and Sphingosine in Fas-induced Apoptosis of Type II Cells-- Abundant reports have suggested that ceramide may play a role in apoptotic signals initiated through the Fas system in various types of cells ( 10- 21, 27, 72).	transcription
71307	3	336167	7	NULL	NULL	0	NULL	Sphingosine	Chemical		play a role in		may			statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_240	10747891	Potential Involvement of Ceramide and Sphingosine in Fas-induced Apoptosis of Type II Cells-- Abundant reports have suggested that ceramide may play a role in apoptotic signals initiated through the Fas system in various types of cells ( 10- 21, 27, 72).	transcription
67080	1	336168	5	NULL	NULL	0	NULL	TNF-alpha	GP		effects					PKCalpha	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29290_s_142	10887171	In an attempt to determine whether ceramide production is necessary for the observed effect of TNF-alpha on PKCalpha, we examined the effect of fumonisin B1, an inhibitor of sphingosine  N-acyltransferase or ceramide synthase ( 30), on PKC activity upon TNF-alpha treatment.	transcription
67081	2	336168	5	NULL	NULL	0	NULL	ceramide	Chemical	production of	is necessary for		potentially			statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29290_s_142	10887171	In an attempt to determine whether ceramide production is necessary for the observed effect of TNF-alpha on PKCalpha, we examined the effect of fumonisin B1, an inhibitor of sphingosine  N-acyltransferase or ceramide synthase ( 30), on PKC activity upon TNF-alpha treatment.	transcription
67082	3	336168	5	NULL	NULL	0	NULL	fumonisin B1	Chemical		is an inhibitor of					sphingosine N-acyltransferase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29290_s_142	10887171	In an attempt to determine whether ceramide production is necessary for the observed effect of TNF-alpha on PKCalpha, we examined the effect of fumonisin B1, an inhibitor of sphingosine  N-acyltransferase or ceramide synthase ( 30), on PKC activity upon TNF-alpha treatment.	transcription
67083	4	336168	5	NULL	NULL	0	NULL	fumonisin B1	Chemical		effects		potentially			PKC	GP	activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29290_s_142	10887171	In an attempt to determine whether ceramide production is necessary for the observed effect of TNF-alpha on PKCalpha, we examined the effect of fumonisin B1, an inhibitor of sphingosine  N-acyltransferase or ceramide synthase ( 30), on PKC activity upon TNF-alpha treatment.	transcription
67084	5	336168	5	NULL	NULL	0	NULL	statement 4	Process		occurs upon					TNF-alpha	GP	treatment			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29290_s_142	10887171	In an attempt to determine whether ceramide production is necessary for the observed effect of TNF-alpha on PKCalpha, we examined the effect of fumonisin B1, an inhibitor of sphingosine  N-acyltransferase or ceramide synthase ( 30), on PKC activity upon TNF-alpha treatment.	transcription
67085	6	336168	5	NULL	NULL	0	NULL	ceramide synthase	GP		effects		potentially			PKC	GP	activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29290_s_142	10887171	In an attempt to determine whether ceramide production is necessary for the observed effect of TNF-alpha on PKCalpha, we examined the effect of fumonisin B1, an inhibitor of sphingosine  N-acyltransferase or ceramide synthase ( 30), on PKC activity upon TNF-alpha treatment.	transcription
67086	7	336168	5	NULL	NULL	0	NULL	statement 6	Process		occurs upon					TNF-alpha	GP	treatment			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29290_s_142	10887171	In an attempt to determine whether ceramide production is necessary for the observed effect of TNF-alpha on PKCalpha, we examined the effect of fumonisin B1, an inhibitor of sphingosine  N-acyltransferase or ceramide synthase ( 30), on PKC activity upon TNF-alpha treatment.	transcription
71308	1	336168	7	NULL	NULL	0	NULL	fumonisin B1	Chemical		inhibit					sphingosine N-acyltransferase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29290_s_142	10887171	In an attempt to determine whether ceramide production is necessary for the observed effect of TNF-alpha on PKCalpha, we examined the effect of fumonisin B1, an inhibitor of sphingosine  N-acyltransferase or ceramide synthase ( 30), on PKC activity upon TNF-alpha treatment.	transcription
71309	2	336168	7	NULL	NULL	0	NULL	fumonisin B1	Chemical		inhibit					ceramide synthase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_38_29290_s_142	10887171	In an attempt to determine whether ceramide production is necessary for the observed effect of TNF-alpha on PKCalpha, we examined the effect of fumonisin B1, an inhibitor of sphingosine  N-acyltransferase or ceramide synthase ( 30), on PKC activity upon TNF-alpha treatment.	transcription
67087	1	336169	5	NULL	NULL	0	NULL	apoptosis	Process		is induced by					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_4_2502_s_217	9891021	Effects of Ceramide Analogs and AHR Ligands on Ceramide induced Apoptosis-- Dihydro- N-acetyl-D- erythro-sphingosine (DHC2-ceramide) differs from C2-ceramide in only one respect; it lacks the double bond between carbons 4 and 5 of the sphingoid backbone.	transcription
67088	2	336169	5	NULL	NULL	0	NULL	ceramide analogs	Chemical		effects					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_4_2502_s_217	9891021	Effects of Ceramide Analogs and AHR Ligands on Ceramide induced Apoptosis-- Dihydro- N-acetyl-D- erythro-sphingosine (DHC2-ceramide) differs from C2-ceramide in only one respect; it lacks the double bond between carbons 4 and 5 of the sphingoid backbone.	transcription
67089	3	336169	5	NULL	NULL	0	NULL	AHR Ligands	Chemical		effects					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_4_2502_s_217	9891021	Effects of Ceramide Analogs and AHR Ligands on Ceramide induced Apoptosis-- Dihydro- N-acetyl-D- erythro-sphingosine (DHC2-ceramide) differs from C2-ceramide in only one respect; it lacks the double bond between carbons 4 and 5 of the sphingoid backbone.	transcription
67090	4	336169	5	NULL	NULL	0	NULL	DHC2-ceramide	Chemical		is					Dihydro- N-acetyl-D- erythro-sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_4_2502_s_217	9891021	Effects of Ceramide Analogs and AHR Ligands on Ceramide induced Apoptosis-- Dihydro- N-acetyl-D- erythro-sphingosine (DHC2-ceramide) differs from C2-ceramide in only one respect; it lacks the double bond between carbons 4 and 5 of the sphingoid backbone.	transcription
71310	1	336169	7	NULL	NULL	0	NULL	ceramide	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_4_2502_s_217	9891021	Effects of Ceramide Analogs and AHR Ligands on Ceramide induced Apoptosis-- Dihydro- N-acetyl-D- erythro-sphingosine (DHC2-ceramide) differs from C2-ceramide in only one respect; it lacks the double bond between carbons 4 and 5 of the sphingoid backbone.	transcription
71311	2	336169	7	NULL	NULL	0	NULL	DHC2-ceramide	Chemical		differs from					C2-ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_4_2502_s_217	9891021	Effects of Ceramide Analogs and AHR Ligands on Ceramide induced Apoptosis-- Dihydro- N-acetyl-D- erythro-sphingosine (DHC2-ceramide) differs from C2-ceramide in only one respect; it lacks the double bond between carbons 4 and 5 of the sphingoid backbone.	transcription
71312	3	336169	7	NULL	NULL	0	NULL	statement 2	Process		lacks 					sphingoid backbone	Chemical	double bond between carbons 4 and 5 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_4_2502_s_217	9891021	Effects of Ceramide Analogs and AHR Ligands on Ceramide induced Apoptosis-- Dihydro- N-acetyl-D- erythro-sphingosine (DHC2-ceramide) differs from C2-ceramide in only one respect; it lacks the double bond between carbons 4 and 5 of the sphingoid backbone.	transcription
71313	4	336169	7	NULL	NULL	0	NULL	DHC2-ceramide	Chemical		is					Dihydro- N-acetyl-D- erythro-sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_4_2502_s_217	9891021	Effects of Ceramide Analogs and AHR Ligands on Ceramide induced Apoptosis-- Dihydro- N-acetyl-D- erythro-sphingosine (DHC2-ceramide) differs from C2-ceramide in only one respect; it lacks the double bond between carbons 4 and 5 of the sphingoid backbone.	transcription
67091	1	336170	5	NULL	NULL	0	NULL	TNFalpha	GP		produce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_146	8981934	Because it has been demonstrated that TNFalpha may produce apoptosis in a variety of cell types, principally through  ceramide production ( 18,  19) or via ceramide's conversion  product, sphingosine ( 20), it is possible that TNFalpha-mediated  cardiac apoptosis may result from enhanced sphingolipid production.	transcription
67092	2	336170	5	NULL	NULL	0	NULL	statement 1	Process		through		principally			ceramide	Chemical	production of			NULL		0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_146	8981934	Because it has been demonstrated that TNFalpha may produce apoptosis in a variety of cell types, principally through  ceramide production ( 18,  19) or via ceramide's conversion  product, sphingosine ( 20), it is possible that TNFalpha-mediated  cardiac apoptosis may result from enhanced sphingolipid production.	transcription
67093	3	336170	5	NULL	NULL	0	NULL	statement 1	Process		via					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_146	8981934	Because it has been demonstrated that TNFalpha may produce apoptosis in a variety of cell types, principally through  ceramide production ( 18,  19) or via ceramide's conversion  product, sphingosine ( 20), it is possible that TNFalpha-mediated  cardiac apoptosis may result from enhanced sphingolipid production.	transcription
67094	4	336170	5	NULL	NULL	0	NULL	sphingosine	Chemical		is a conversion product of					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_146	8981934	Because it has been demonstrated that TNFalpha may produce apoptosis in a variety of cell types, principally through  ceramide production ( 18,  19) or via ceramide's conversion  product, sphingosine ( 20), it is possible that TNFalpha-mediated  cardiac apoptosis may result from enhanced sphingolipid production.	transcription
67095	5	336170	5	NULL	NULL	0	NULL	TNFalpha	GP		mediates					apoptosis	Process	cardiac			NULL		0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_146	8981934	Because it has been demonstrated that TNFalpha may produce apoptosis in a variety of cell types, principally through  ceramide production ( 18,  19) or via ceramide's conversion  product, sphingosine ( 20), it is possible that TNFalpha-mediated  cardiac apoptosis may result from enhanced sphingolipid production.	transcription
67096	6	336170	5	NULL	NULL	0	NULL	statement 5	Process		results from		may			sphingosine	Chemical	enhanced production of			NULL		0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_146	8981934	Because it has been demonstrated that TNFalpha may produce apoptosis in a variety of cell types, principally through  ceramide production ( 18,  19) or via ceramide's conversion  product, sphingosine ( 20), it is possible that TNFalpha-mediated  cardiac apoptosis may result from enhanced sphingolipid production.	transcription
71314	1	336170	7	NULL	NULL	0	NULL	TNFalpha	GP		produce		may			apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_146	8981934	Because it has been demonstrated that TNFalpha may produce apoptosis in a variety of cell types, principally through  ceramide production ( 18,  19) or via ceramide's conversion  product, sphingosine ( 20), it is possible that TNFalpha-mediated  cardiac apoptosis may result from enhanced sphingolipid production.	transcription
71315	2	336170	7	NULL	NULL	0	NULL	statement 1	Process		occur through					ceramide	Chemical	production of			NULL		0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_146	8981934	Because it has been demonstrated that TNFalpha may produce apoptosis in a variety of cell types, principally through  ceramide production ( 18,  19) or via ceramide's conversion  product, sphingosine ( 20), it is possible that TNFalpha-mediated  cardiac apoptosis may result from enhanced sphingolipid production.	transcription
71316	3	336170	7	NULL	NULL	0	NULL	statement 1	Process		occur through					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_146	8981934	Because it has been demonstrated that TNFalpha may produce apoptosis in a variety of cell types, principally through  ceramide production ( 18,  19) or via ceramide's conversion  product, sphingosine ( 20), it is possible that TNFalpha-mediated  cardiac apoptosis may result from enhanced sphingolipid production.	transcription
71317	4	336170	7	NULL	NULL	0	NULL	sphingosine	Chemical		is a type of					ceramide conversion product	Chemical				NULL		0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_146	8981934	Because it has been demonstrated that TNFalpha may produce apoptosis in a variety of cell types, principally through  ceramide production ( 18,  19) or via ceramide's conversion  product, sphingosine ( 20), it is possible that TNFalpha-mediated  cardiac apoptosis may result from enhanced sphingolipid production.	transcription
71318	5	336170	7	NULL	NULL	0	NULL	TNFalpha	GP		mediates					cardiac apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_146	8981934	Because it has been demonstrated that TNFalpha may produce apoptosis in a variety of cell types, principally through  ceramide production ( 18,  19) or via ceramide's conversion  product, sphingosine ( 20), it is possible that TNFalpha-mediated  cardiac apoptosis may result from enhanced sphingolipid production.	transcription
71319	6	336170	7	NULL	NULL	0	NULL	statement 5	Process		result from		may			sphingolipid	Chemical	enhanced production of			NULL		0	NULL	NULL	NULL	gw60_jclininvest_98_12_2854_s_146	8981934	Because it has been demonstrated that TNFalpha may produce apoptosis in a variety of cell types, principally through  ceramide production ( 18,  19) or via ceramide's conversion  product, sphingosine ( 20), it is possible that TNFalpha-mediated  cardiac apoptosis may result from enhanced sphingolipid production.	transcription
67097	1	336171	5	NULL	NULL	0	NULL	SPHK1	GP	enforced expression of 	increases		significantly			SPHK1	GP	kinase activity of			NULL	PC12 cells	0	NULL	NULL	NULL	abs-batch0650-0679_j-neurochem_76_5_11238741_s_5	11238741	Enforced expression of SPHK1 in PC12  cells resulted in significant increases in kinase activity, with corresponding  increases in intracellular SPP levels and concomitant decreases in both  sphingosine and ceramide, and marked suppression of apoptosis induced  by trophic factor withdrawal or by C(2)-ceramide.	transcription
67098	2	336171	5	NULL	NULL	0	NULL	statement 1	Process		increases					SPP	Chemical	intracellular levels of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-neurochem_76_5_11238741_s_5	11238741	Enforced expression of SPHK1 in PC12  cells resulted in significant increases in kinase activity, with corresponding  increases in intracellular SPP levels and concomitant decreases in both  sphingosine and ceramide, and marked suppression of apoptosis induced  by trophic factor withdrawal or by C(2)-ceramide.	transcription
67099	3	336171	5	NULL	NULL	0	NULL	statement 1	Process		decreases					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-neurochem_76_5_11238741_s_5	11238741	Enforced expression of SPHK1 in PC12  cells resulted in significant increases in kinase activity, with corresponding  increases in intracellular SPP levels and concomitant decreases in both  sphingosine and ceramide, and marked suppression of apoptosis induced  by trophic factor withdrawal or by C(2)-ceramide.	transcription
67100	4	336171	5	NULL	NULL	0	NULL	statement 1	Process		decreases					ceramide	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-neurochem_76_5_11238741_s_5	11238741	Enforced expression of SPHK1 in PC12  cells resulted in significant increases in kinase activity, with corresponding  increases in intracellular SPP levels and concomitant decreases in both  sphingosine and ceramide, and marked suppression of apoptosis induced  by trophic factor withdrawal or by C(2)-ceramide.	transcription
67101	5	336171	5	NULL	NULL	0	NULL	statement 3	Process		is concomitant to					statement 2	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-neurochem_76_5_11238741_s_5	11238741	Enforced expression of SPHK1 in PC12  cells resulted in significant increases in kinase activity, with corresponding  increases in intracellular SPP levels and concomitant decreases in both  sphingosine and ceramide, and marked suppression of apoptosis induced  by trophic factor withdrawal or by C(2)-ceramide.	transcription
67102	6	336171	5	NULL	NULL	0	NULL	statement 4	Process		is concomitant to					statement 2	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-neurochem_76_5_11238741_s_5	11238741	Enforced expression of SPHK1 in PC12  cells resulted in significant increases in kinase activity, with corresponding  increases in intracellular SPP levels and concomitant decreases in both  sphingosine and ceramide, and marked suppression of apoptosis induced  by trophic factor withdrawal or by C(2)-ceramide.	transcription
67103	7	336171	5	NULL	NULL	0	NULL	apoptosis	Process		is induced by					trophic factor	GP	withdrawal of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-neurochem_76_5_11238741_s_5	11238741	Enforced expression of SPHK1 in PC12  cells resulted in significant increases in kinase activity, with corresponding  increases in intracellular SPP levels and concomitant decreases in both  sphingosine and ceramide, and marked suppression of apoptosis induced  by trophic factor withdrawal or by C(2)-ceramide.	transcription
67104	8	336171	5	NULL	NULL	0	NULL	apoptosis	Process		is induced by					C(2)-ceramide	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-neurochem_76_5_11238741_s_5	11238741	Enforced expression of SPHK1 in PC12  cells resulted in significant increases in kinase activity, with corresponding  increases in intracellular SPP levels and concomitant decreases in both  sphingosine and ceramide, and marked suppression of apoptosis induced  by trophic factor withdrawal or by C(2)-ceramide.	transcription
67105	9	336171	5	NULL	NULL	0	NULL	statement 7	Process		is an alternative to					statement 8	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-neurochem_76_5_11238741_s_5	11238741	Enforced expression of SPHK1 in PC12  cells resulted in significant increases in kinase activity, with corresponding  increases in intracellular SPP levels and concomitant decreases in both  sphingosine and ceramide, and marked suppression of apoptosis induced  by trophic factor withdrawal or by C(2)-ceramide.	transcription
67106	10	336171	5	NULL	NULL	0	NULL	statement 1	Process		suppress					statement 7	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-neurochem_76_5_11238741_s_5	11238741	Enforced expression of SPHK1 in PC12  cells resulted in significant increases in kinase activity, with corresponding  increases in intracellular SPP levels and concomitant decreases in both  sphingosine and ceramide, and marked suppression of apoptosis induced  by trophic factor withdrawal or by C(2)-ceramide.	transcription
67107	11	336171	5	NULL	NULL	0	NULL	statement 1	Process		suppress					statement 8	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-neurochem_76_5_11238741_s_5	11238741	Enforced expression of SPHK1 in PC12  cells resulted in significant increases in kinase activity, with corresponding  increases in intracellular SPP levels and concomitant decreases in both  sphingosine and ceramide, and marked suppression of apoptosis induced  by trophic factor withdrawal or by C(2)-ceramide.	transcription
71320	1	336171	7	NULL	NULL	0	NULL	SPHK1	GP		increase		significantly			kinase activity	Process				NULL	PC12 cells	0	NULL	NULL	NULL	abs-batch0650-0679_j-neurochem_76_5_11238741_s_5	11238741	Enforced expression of SPHK1 in PC12  cells resulted in significant increases in kinase activity, with corresponding  increases in intracellular SPP levels and concomitant decreases in both  sphingosine and ceramide, and marked suppression of apoptosis induced  by trophic factor withdrawal or by C(2)-ceramide.	transcription
71321	2	336171	7	NULL	NULL	NULL	NULL	statement 1	Process		increase		correspondingly			SPP	Chemical	intracellular			NULL	PC12 cells	NULL	NULL	NULL	NULL	abs-batch0650-0679_j-neurochem_76_5_11238741_s_5	11238741	Enforced expression of SPHK1 in PC12  cells resulted in significant increases in kinase activity, with corresponding  increases in intracellular SPP levels and concomitant decreases in both  sphingosine and ceramide, and marked suppression of apoptosis induced  by trophic factor withdrawal or by C(2)-ceramide.	transcription
71322	3	336171	7	NULL	NULL	NULL	NULL	statement 1	Process		decrease		concomitantly			sphingosine	Chemical				NULL	PC12 cells	NULL	NULL	NULL	NULL	abs-batch0650-0679_j-neurochem_76_5_11238741_s_5	11238741	Enforced expression of SPHK1 in PC12  cells resulted in significant increases in kinase activity, with corresponding  increases in intracellular SPP levels and concomitant decreases in both  sphingosine and ceramide, and marked suppression of apoptosis induced  by trophic factor withdrawal or by C(2)-ceramide.	transcription
71323	4	336171	7	NULL	NULL	NULL	NULL	statement 1	Process		decrease		concomitantly			ceramide	Chemical				NULL	PC12 cells	NULL	NULL	NULL	NULL	abs-batch0650-0679_j-neurochem_76_5_11238741_s_5	11238741	Enforced expression of SPHK1 in PC12  cells resulted in significant increases in kinase activity, with corresponding  increases in intracellular SPP levels and concomitant decreases in both  sphingosine and ceramide, and marked suppression of apoptosis induced  by trophic factor withdrawal or by C(2)-ceramide.	transcription
71324	5	336171	7	NULL	NULL	NULL	NULL	trophic factor	GP	withdrawal of	induce					apoptosis	Process				NULL	PC12 cells	NULL	NULL	NULL	NULL	abs-batch0650-0679_j-neurochem_76_5_11238741_s_5	11238741	Enforced expression of SPHK1 in PC12  cells resulted in significant increases in kinase activity, with corresponding  increases in intracellular SPP levels and concomitant decreases in both  sphingosine and ceramide, and marked suppression of apoptosis induced  by trophic factor withdrawal or by C(2)-ceramide.	transcription
71325	6	336171	7	NULL	NULL	NULL	NULL	C(2)-ceramide	Chemical		induce					apoptosis	Process				NULL	PC12 cells	NULL	NULL	NULL	NULL	abs-batch0650-0679_j-neurochem_76_5_11238741_s_5	11238741	Enforced expression of SPHK1 in PC12  cells resulted in significant increases in kinase activity, with corresponding  increases in intracellular SPP levels and concomitant decreases in both  sphingosine and ceramide, and marked suppression of apoptosis induced  by trophic factor withdrawal or by C(2)-ceramide.	transcription
71326	7	336171	7	NULL	NULL	NULL	NULL	SPHK1	GP		suppress		markedly			statement 5	Process				NULL	PC12 cells	NULL	NULL	NULL	NULL	abs-batch0650-0679_j-neurochem_76_5_11238741_s_5	11238741	Enforced expression of SPHK1 in PC12  cells resulted in significant increases in kinase activity, with corresponding  increases in intracellular SPP levels and concomitant decreases in both  sphingosine and ceramide, and marked suppression of apoptosis induced  by trophic factor withdrawal or by C(2)-ceramide.	transcription
71327	8	336171	7	NULL	NULL	NULL	NULL	SPHK1	GP		suppress		markedly			statement 6	Process				NULL	PC12 cells	NULL	NULL	NULL	NULL	abs-batch0650-0679_j-neurochem_76_5_11238741_s_5	11238741	Enforced expression of SPHK1 in PC12  cells resulted in significant increases in kinase activity, with corresponding  increases in intracellular SPP levels and concomitant decreases in both  sphingosine and ceramide, and marked suppression of apoptosis induced  by trophic factor withdrawal or by C(2)-ceramide.	transcription
67108	1	336172	5	NULL	NULL	0	NULL	long chain ceramide	Chemical	sustained generation of;;endogenous	requires					C6-ceramide	Chemical	biochemical recycling of;;sphingosine backbone of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12960_s_37	11815611	We show here, for the first time, that the sustained generation of long chain endogenous ceramide requires the biochemical recycling of the sphingosine backbone of C6-ceramide, which involves deacylation and reacylation of ceramide for the generation of endogenous long chain ceramide (mainly C16:0- and C24:1-ceramides), most likely by CoA-dependent ceramide synthase, which is inhibited by fumonisin B1.	transcription
67109	2	336172	5	NULL	NULL	0	NULL	C6-ceramide	Chemical	biochemical recycling of;;sphingosine backbone of	involves					ceramide	Chemical	deacylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12960_s_37	11815611	We show here, for the first time, that the sustained generation of long chain endogenous ceramide requires the biochemical recycling of the sphingosine backbone of C6-ceramide, which involves deacylation and reacylation of ceramide for the generation of endogenous long chain ceramide (mainly C16:0- and C24:1-ceramides), most likely by CoA-dependent ceramide synthase, which is inhibited by fumonisin B1.	transcription
67110	3	336172	5	NULL	NULL	0	NULL	C6-ceramide	Chemical	biochemical recycling of;;sphingosine backbone of	involves					ceramide	Chemical	reacylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12960_s_37	11815611	We show here, for the first time, that the sustained generation of long chain endogenous ceramide requires the biochemical recycling of the sphingosine backbone of C6-ceramide, which involves deacylation and reacylation of ceramide for the generation of endogenous long chain ceramide (mainly C16:0- and C24:1-ceramides), most likely by CoA-dependent ceramide synthase, which is inhibited by fumonisin B1.	transcription
67111	4	336172	5	NULL	NULL	0	NULL	statement 2	Process		occurs along with					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12960_s_37	11815611	We show here, for the first time, that the sustained generation of long chain endogenous ceramide requires the biochemical recycling of the sphingosine backbone of C6-ceramide, which involves deacylation and reacylation of ceramide for the generation of endogenous long chain ceramide (mainly C16:0- and C24:1-ceramides), most likely by CoA-dependent ceramide synthase, which is inhibited by fumonisin B1.	transcription
67112	5	336172	5	NULL	NULL	0	NULL	statement 4	Process		generates					long chain ceramide	Chemical	endogenous			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12960_s_37	11815611	We show here, for the first time, that the sustained generation of long chain endogenous ceramide requires the biochemical recycling of the sphingosine backbone of C6-ceramide, which involves deacylation and reacylation of ceramide for the generation of endogenous long chain ceramide (mainly C16:0- and C24:1-ceramides), most likely by CoA-dependent ceramide synthase, which is inhibited by fumonisin B1.	transcription
67113	6	336172	5	NULL	NULL	0	NULL	C24:1-ceramide	Chemical		is a type of					long chain ceramide					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12960_s_37	11815611	We show here, for the first time, that the sustained generation of long chain endogenous ceramide requires the biochemical recycling of the sphingosine backbone of C6-ceramide, which involves deacylation and reacylation of ceramide for the generation of endogenous long chain ceramide (mainly C16:0- and C24:1-ceramides), most likely by CoA-dependent ceramide synthase, which is inhibited by fumonisin B1.	transcription
67114	7	336172	5	NULL	NULL	0	NULL	C16:0-ceramide	Chemical		is a type of					long chain ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12960_s_37	11815611	We show here, for the first time, that the sustained generation of long chain endogenous ceramide requires the biochemical recycling of the sphingosine backbone of C6-ceramide, which involves deacylation and reacylation of ceramide for the generation of endogenous long chain ceramide (mainly C16:0- and C24:1-ceramides), most likely by CoA-dependent ceramide synthase, which is inhibited by fumonisin B1.	transcription
67115	8	336172	5	NULL	NULL	0	NULL	ceramide synthase	GP		is dependent on					CoA	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12960_s_37	11815611	We show here, for the first time, that the sustained generation of long chain endogenous ceramide requires the biochemical recycling of the sphingosine backbone of C6-ceramide, which involves deacylation and reacylation of ceramide for the generation of endogenous long chain ceramide (mainly C16:0- and C24:1-ceramides), most likely by CoA-dependent ceramide synthase, which is inhibited by fumonisin B1.	transcription
67116	9	336172	5	NULL	NULL	0	NULL	ceramide synthase	GP		catalyzes					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12960_s_37	11815611	We show here, for the first time, that the sustained generation of long chain endogenous ceramide requires the biochemical recycling of the sphingosine backbone of C6-ceramide, which involves deacylation and reacylation of ceramide for the generation of endogenous long chain ceramide (mainly C16:0- and C24:1-ceramides), most likely by CoA-dependent ceramide synthase, which is inhibited by fumonisin B1.	transcription
67117	10	336172	5	NULL	NULL	0	NULL	ceramide synthase	GP		catalyzes					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12960_s_37	11815611	We show here, for the first time, that the sustained generation of long chain endogenous ceramide requires the biochemical recycling of the sphingosine backbone of C6-ceramide, which involves deacylation and reacylation of ceramide for the generation of endogenous long chain ceramide (mainly C16:0- and C24:1-ceramides), most likely by CoA-dependent ceramide synthase, which is inhibited by fumonisin B1.	transcription
67118	11	336172	5	NULL	NULL	0	NULL	fumonisin B1	Chemical		inhibits					ceramide synthase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12960_s_37	11815611	We show here, for the first time, that the sustained generation of long chain endogenous ceramide requires the biochemical recycling of the sphingosine backbone of C6-ceramide, which involves deacylation and reacylation of ceramide for the generation of endogenous long chain ceramide (mainly C16:0- and C24:1-ceramides), most likely by CoA-dependent ceramide synthase, which is inhibited by fumonisin B1.	transcription
71328	1	336172	7	NULL	NULL	0	NULL	long chain ceramide	Chemical	sustained generation of ;;endogenous 	requires					C6-ceramide	Chemical	biochemical recycling of;;sphingosine backbone of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12960_s_37	11815611	We show here, for the first time, that the sustained generation of long chain endogenous ceramide requires the biochemical recycling of the sphingosine backbone of C6-ceramide, which involves deacylation and reacylation of ceramide for the generation of endogenous long chain ceramide (mainly C16:0- and C24:1-ceramides), most likely by CoA-dependent ceramide synthase, which is inhibited by fumonisin B1.	transcription
71329	2	336172	7	NULL	NULL	NULL	NULL	C6-ceramide	Chemical	biochemical recycling of	involves					ceramide	Chemical	deacylation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_12960_s_37	11815611	We show here, for the first time, that the sustained generation of long chain endogenous ceramide requires the biochemical recycling of the sphingosine backbone of C6-ceramide, which involves deacylation and reacylation of ceramide for the generation of endogenous long chain ceramide (mainly C16:0- and C24:1-ceramides), most likely by CoA-dependent ceramide synthase, which is inhibited by fumonisin B1.	transcription
71330	3	336172	7	NULL	NULL	0	NULL	C6-ceramide	Chemical	biochemical recycling of	involves					ceramide	Chemical	reacylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12960_s_37	11815611	We show here, for the first time, that the sustained generation of long chain endogenous ceramide requires the biochemical recycling of the sphingosine backbone of C6-ceramide, which involves deacylation and reacylation of ceramide for the generation of endogenous long chain ceramide (mainly C16:0- and C24:1-ceramides), most likely by CoA-dependent ceramide synthase, which is inhibited by fumonisin B1.	transcription
71331	4	336172	7	NULL	NULL	0	NULL	statement 2	Process		occur along with					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12960_s_37	11815611	We show here, for the first time, that the sustained generation of long chain endogenous ceramide requires the biochemical recycling of the sphingosine backbone of C6-ceramide, which involves deacylation and reacylation of ceramide for the generation of endogenous long chain ceramide (mainly C16:0- and C24:1-ceramides), most likely by CoA-dependent ceramide synthase, which is inhibited by fumonisin B1.	transcription
71332	5	336172	7	NULL	NULL	NULL	NULL	statement 4	Process		generate					C16:0 ceramide	Chemical	endogenous;;long chain			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_12960_s_37	11815611	We show here, for the first time, that the sustained generation of long chain endogenous ceramide requires the biochemical recycling of the sphingosine backbone of C6-ceramide, which involves deacylation and reacylation of ceramide for the generation of endogenous long chain ceramide (mainly C16:0- and C24:1-ceramides), most likely by CoA-dependent ceramide synthase, which is inhibited by fumonisin B1.	transcription
71333	6	336172	7	NULL	NULL	NULL	NULL	statement 4	Process		generate					C24:1ceramide	Chemical	endogenous;;long chain			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_12960_s_37	11815611	We show here, for the first time, that the sustained generation of long chain endogenous ceramide requires the biochemical recycling of the sphingosine backbone of C6-ceramide, which involves deacylation and reacylation of ceramide for the generation of endogenous long chain ceramide (mainly C16:0- and C24:1-ceramides), most likely by CoA-dependent ceramide synthase, which is inhibited by fumonisin B1.	transcription
71334	7	336172	7	NULL	NULL	0	NULL	CoA-dependent ceramide synthase	GP		catalyze					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12960_s_37	11815611	We show here, for the first time, that the sustained generation of long chain endogenous ceramide requires the biochemical recycling of the sphingosine backbone of C6-ceramide, which involves deacylation and reacylation of ceramide for the generation of endogenous long chain ceramide (mainly C16:0- and C24:1-ceramides), most likely by CoA-dependent ceramide synthase, which is inhibited by fumonisin B1.	transcription
71335	8	336172	7	NULL	NULL	0	NULL	fumonisin B1	Chemical		inhibit					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12960_s_37	11815611	We show here, for the first time, that the sustained generation of long chain endogenous ceramide requires the biochemical recycling of the sphingosine backbone of C6-ceramide, which involves deacylation and reacylation of ceramide for the generation of endogenous long chain ceramide (mainly C16:0- and C24:1-ceramides), most likely by CoA-dependent ceramide synthase, which is inhibited by fumonisin B1.	transcription
67198	1	336173	5	NULL	NULL	NULL	NULL	sphingomyelinase	GP	bacterial	generates					ceramide	Chemical				NULL	plasma membrane	NULL	NULL	NULL	NULL	gw60_science_274_5294_1855_s_69	8943189	For example, the addition of precursor gangliosides, precursor sphingosine, bacterial sphingomyelinase (which generates ceramide at the plasma membrane), D- threo-1-phenyl-2-decanoylamino-3-morpholino- 1-propanol (PDMP) (which inhibits further incorporation of ceramide into glycolipids), or D- erythro-2-( N-myristoylamino)-1-phenyl-1-propanol (D-MAPP) (which inhibits ceramide metabolism through ceramidase) results in accumulation of ceramide ranging from three to eight times the concentrations in unstimulated cells ( 19).	transcription
67199	2	336173	5	NULL	NULL	0	NULL	PDMP3	Chemical		is					D- threo-1-phenyl-2-decanoylamino-3-morpholino- 1-propanol	Chemical				NULL		0	NULL	NULL	NULL	gw60_science_274_5294_1855_s_69	8943189	For example, the addition of precursor gangliosides, precursor sphingosine, bacterial sphingomyelinase (which generates ceramide at the plasma membrane), D- threo-1-phenyl-2-decanoylamino-3-morpholino- 1-propanol (PDMP) (which inhibits further incorporation of ceramide into glycolipids), or D- erythro-2-( N-myristoylamino)-1-phenyl-1-propanol (D-MAPP) (which inhibits ceramide metabolism through ceramidase) results in accumulation of ceramide ranging from three to eight times the concentrations in unstimulated cells ( 19).	transcription
67200	3	336173	5	NULL	NULL	0	NULL	ceramide	Chemical		is incorporated into					glycolipids	Chemical				NULL		0	NULL	NULL	NULL	gw60_science_274_5294_1855_s_69	8943189	For example, the addition of precursor gangliosides, precursor sphingosine, bacterial sphingomyelinase (which generates ceramide at the plasma membrane), D- threo-1-phenyl-2-decanoylamino-3-morpholino- 1-propanol (PDMP) (which inhibits further incorporation of ceramide into glycolipids), or D- erythro-2-( N-myristoylamino)-1-phenyl-1-propanol (D-MAPP) (which inhibits ceramide metabolism through ceramidase) results in accumulation of ceramide ranging from three to eight times the concentrations in unstimulated cells ( 19).	transcription
67201	4	336173	5	NULL	NULL	0	NULL	PDMP	Chemical		inhibits					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_science_274_5294_1855_s_69	8943189	For example, the addition of precursor gangliosides, precursor sphingosine, bacterial sphingomyelinase (which generates ceramide at the plasma membrane), D- threo-1-phenyl-2-decanoylamino-3-morpholino- 1-propanol (PDMP) (which inhibits further incorporation of ceramide into glycolipids), or D- erythro-2-( N-myristoylamino)-1-phenyl-1-propanol (D-MAPP) (which inhibits ceramide metabolism through ceramidase) results in accumulation of ceramide ranging from three to eight times the concentrations in unstimulated cells ( 19).	transcription
67202	5	336173	5	NULL	NULL	0	NULL	D-MAPP	Chemical		is					D- erythro-2-( N-myristoylamino)-1-phenyl-1-propanol	Chemical				NULL		0	NULL	NULL	NULL	gw60_science_274_5294_1855_s_69	8943189	For example, the addition of precursor gangliosides, precursor sphingosine, bacterial sphingomyelinase (which generates ceramide at the plasma membrane), D- threo-1-phenyl-2-decanoylamino-3-morpholino- 1-propanol (PDMP) (which inhibits further incorporation of ceramide into glycolipids), or D- erythro-2-( N-myristoylamino)-1-phenyl-1-propanol (D-MAPP) (which inhibits ceramide metabolism through ceramidase) results in accumulation of ceramide ranging from three to eight times the concentrations in unstimulated cells ( 19).	transcription
67203	6	336173	5	NULL	NULL	0	NULL	ceramide	Chemical	metabolism of	occurs through					ceramidase	GP				NULL		0	NULL	NULL	NULL	gw60_science_274_5294_1855_s_69	8943189	For example, the addition of precursor gangliosides, precursor sphingosine, bacterial sphingomyelinase (which generates ceramide at the plasma membrane), D- threo-1-phenyl-2-decanoylamino-3-morpholino- 1-propanol (PDMP) (which inhibits further incorporation of ceramide into glycolipids), or D- erythro-2-( N-myristoylamino)-1-phenyl-1-propanol (D-MAPP) (which inhibits ceramide metabolism through ceramidase) results in accumulation of ceramide ranging from three to eight times the concentrations in unstimulated cells ( 19).	transcription
67204	7	336173	5	NULL	NULL	0	NULL	D-MAPP	Chemical		inhibits					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_science_274_5294_1855_s_69	8943189	For example, the addition of precursor gangliosides, precursor sphingosine, bacterial sphingomyelinase (which generates ceramide at the plasma membrane), D- threo-1-phenyl-2-decanoylamino-3-morpholino- 1-propanol (PDMP) (which inhibits further incorporation of ceramide into glycolipids), or D- erythro-2-( N-myristoylamino)-1-phenyl-1-propanol (D-MAPP) (which inhibits ceramide metabolism through ceramidase) results in accumulation of ceramide ranging from three to eight times the concentrations in unstimulated cells ( 19).	transcription
67205	8	336173	5	NULL	NULL	0	NULL	ganglioside precursor	Chemical	addition of	results in					ceramide	Chemical	accumulation of			NULL		0	NULL	NULL	NULL	gw60_science_274_5294_1855_s_69	8943189	For example, the addition of precursor gangliosides, precursor sphingosine, bacterial sphingomyelinase (which generates ceramide at the plasma membrane), D- threo-1-phenyl-2-decanoylamino-3-morpholino- 1-propanol (PDMP) (which inhibits further incorporation of ceramide into glycolipids), or D- erythro-2-( N-myristoylamino)-1-phenyl-1-propanol (D-MAPP) (which inhibits ceramide metabolism through ceramidase) results in accumulation of ceramide ranging from three to eight times the concentrations in unstimulated cells ( 19).	transcription
67206	9	336173	5	NULL	NULL	0	NULL	sphingosine precursor	Chemical	addition of	results in					ceramide	Chemical	accumulation of			NULL		0	NULL	NULL	NULL	gw60_science_274_5294_1855_s_69	8943189	For example, the addition of precursor gangliosides, precursor sphingosine, bacterial sphingomyelinase (which generates ceramide at the plasma membrane), D- threo-1-phenyl-2-decanoylamino-3-morpholino- 1-propanol (PDMP) (which inhibits further incorporation of ceramide into glycolipids), or D- erythro-2-( N-myristoylamino)-1-phenyl-1-propanol (D-MAPP) (which inhibits ceramide metabolism through ceramidase) results in accumulation of ceramide ranging from three to eight times the concentrations in unstimulated cells ( 19).	transcription
67207	10	336173	5	NULL	NULL	0	NULL	sphingomyelinase	GP	addition of;;bacterial	results in					ceramide	Chemical	accumulation of			NULL		0	NULL	NULL	NULL	gw60_science_274_5294_1855_s_69	8943189	For example, the addition of precursor gangliosides, precursor sphingosine, bacterial sphingomyelinase (which generates ceramide at the plasma membrane), D- threo-1-phenyl-2-decanoylamino-3-morpholino- 1-propanol (PDMP) (which inhibits further incorporation of ceramide into glycolipids), or D- erythro-2-( N-myristoylamino)-1-phenyl-1-propanol (D-MAPP) (which inhibits ceramide metabolism through ceramidase) results in accumulation of ceramide ranging from three to eight times the concentrations in unstimulated cells ( 19).	transcription
67208	11	336173	5	NULL	NULL	0	NULL	PDMP	Chemical	addition of	results in					ceramide	Chemical	accumulation of			NULL		0	NULL	NULL	NULL	gw60_science_274_5294_1855_s_69	8943189	For example, the addition of precursor gangliosides, precursor sphingosine, bacterial sphingomyelinase (which generates ceramide at the plasma membrane), D- threo-1-phenyl-2-decanoylamino-3-morpholino- 1-propanol (PDMP) (which inhibits further incorporation of ceramide into glycolipids), or D- erythro-2-( N-myristoylamino)-1-phenyl-1-propanol (D-MAPP) (which inhibits ceramide metabolism through ceramidase) results in accumulation of ceramide ranging from three to eight times the concentrations in unstimulated cells ( 19).	transcription
67209	12	336173	5	NULL	NULL	0	NULL	D-MAPP	Chemical	addition of	results in					ceramide	Chemical	accumulation of			NULL		0	NULL	NULL	NULL	gw60_science_274_5294_1855_s_69	8943189	For example, the addition of precursor gangliosides, precursor sphingosine, bacterial sphingomyelinase (which generates ceramide at the plasma membrane), D- threo-1-phenyl-2-decanoylamino-3-morpholino- 1-propanol (PDMP) (which inhibits further incorporation of ceramide into glycolipids), or D- erythro-2-( N-myristoylamino)-1-phenyl-1-propanol (D-MAPP) (which inhibits ceramide metabolism through ceramidase) results in accumulation of ceramide ranging from three to eight times the concentrations in unstimulated cells ( 19).	transcription
71336	1	336173	7	NULL	NULL	NULL	NULL	precursor gangliosides	Chemical	addition of	results in					ceramide	Chemical	accumulation of			NULL	unstimulated cells	NULL	NULL	NULL	NULL	gw60_science_274_5294_1855_s_69	8943189	For example, the addition of precursor gangliosides, precursor sphingosine, bacterial sphingomyelinase (which generates ceramide at the plasma membrane), D- threo-1-phenyl-2-decanoylamino-3-morpholino- 1-propanol (PDMP) (which inhibits further incorporation of ceramide into glycolipids), or D- erythro-2-( N-myristoylamino)-1-phenyl-1-propanol (D-MAPP) (which inhibits ceramide metabolism through ceramidase) results in accumulation of ceramide ranging from three to eight times the concentrations in unstimulated cells ( 19).	transcription
71337	2	336173	7	NULL	NULL	NULL	NULL	precursor sphingosine	Chemical	addition of	results in					ceramide	Chemical	accumulation of			NULL	unstimulated cells	NULL	NULL	NULL	NULL	gw60_science_274_5294_1855_s_69	8943189	For example, the addition of precursor gangliosides, precursor sphingosine, bacterial sphingomyelinase (which generates ceramide at the plasma membrane), D- threo-1-phenyl-2-decanoylamino-3-morpholino- 1-propanol (PDMP) (which inhibits further incorporation of ceramide into glycolipids), or D- erythro-2-( N-myristoylamino)-1-phenyl-1-propanol (D-MAPP) (which inhibits ceramide metabolism through ceramidase) results in accumulation of ceramide ranging from three to eight times the concentrations in unstimulated cells ( 19).	transcription
71338	3	336173	7	NULL	NULL	0	NULL	sphingomyelinase	GP	bacterial	generates					ceramide	Chemical				NULL	plasma membrane	0	NULL	NULL	NULL	gw60_science_274_5294_1855_s_69	8943189	For example, the addition of precursor gangliosides, precursor sphingosine, bacterial sphingomyelinase (which generates ceramide at the plasma membrane), D- threo-1-phenyl-2-decanoylamino-3-morpholino- 1-propanol (PDMP) (which inhibits further incorporation of ceramide into glycolipids), or D- erythro-2-( N-myristoylamino)-1-phenyl-1-propanol (D-MAPP) (which inhibits ceramide metabolism through ceramidase) results in accumulation of ceramide ranging from three to eight times the concentrations in unstimulated cells ( 19).	transcription
71339	4	336173	7	NULL	NULL	NULL	NULL	sphingomyelinase	GP	bacterial;addition of	results in					ceramide	Chemical	accumulation of			NULL	unstimulated cells	NULL	NULL	NULL	NULL	gw60_science_274_5294_1855_s_69	8943189	For example, the addition of precursor gangliosides, precursor sphingosine, bacterial sphingomyelinase (which generates ceramide at the plasma membrane), D- threo-1-phenyl-2-decanoylamino-3-morpholino- 1-propanol (PDMP) (which inhibits further incorporation of ceramide into glycolipids), or D- erythro-2-( N-myristoylamino)-1-phenyl-1-propanol (D-MAPP) (which inhibits ceramide metabolism through ceramidase) results in accumulation of ceramide ranging from three to eight times the concentrations in unstimulated cells ( 19).	transcription
71340	5	336173	7	NULL	NULL	NULL	NULL	PDMP	Chemical	addition of	results in					ceramide	Chemical	accumulation of			NULL	unstimulated cells	NULL	NULL	NULL	NULL	gw60_science_274_5294_1855_s_69	8943189	For example, the addition of precursor gangliosides, precursor sphingosine, bacterial sphingomyelinase (which generates ceramide at the plasma membrane), D- threo-1-phenyl-2-decanoylamino-3-morpholino- 1-propanol (PDMP) (which inhibits further incorporation of ceramide into glycolipids), or D- erythro-2-( N-myristoylamino)-1-phenyl-1-propanol (D-MAPP) (which inhibits ceramide metabolism through ceramidase) results in accumulation of ceramide ranging from three to eight times the concentrations in unstimulated cells ( 19).	transcription
71341	6	336173	7	NULL	NULL	0	NULL	ceramide	Chemical		incorporated into					glycolipids	Chemical				NULL		0	NULL	NULL	NULL	gw60_science_274_5294_1855_s_69	8943189	For example, the addition of precursor gangliosides, precursor sphingosine, bacterial sphingomyelinase (which generates ceramide at the plasma membrane), D- threo-1-phenyl-2-decanoylamino-3-morpholino- 1-propanol (PDMP) (which inhibits further incorporation of ceramide into glycolipids), or D- erythro-2-( N-myristoylamino)-1-phenyl-1-propanol (D-MAPP) (which inhibits ceramide metabolism through ceramidase) results in accumulation of ceramide ranging from three to eight times the concentrations in unstimulated cells ( 19).	transcription
71342	7	336173	7	NULL	NULL	0	NULL	PDMP	Chemical		inhibit					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_science_274_5294_1855_s_69	8943189	For example, the addition of precursor gangliosides, precursor sphingosine, bacterial sphingomyelinase (which generates ceramide at the plasma membrane), D- threo-1-phenyl-2-decanoylamino-3-morpholino- 1-propanol (PDMP) (which inhibits further incorporation of ceramide into glycolipids), or D- erythro-2-( N-myristoylamino)-1-phenyl-1-propanol (D-MAPP) (which inhibits ceramide metabolism through ceramidase) results in accumulation of ceramide ranging from three to eight times the concentrations in unstimulated cells ( 19).	transcription
71343	8	336173	7	NULL	NULL	0	NULL	PDMP	Chemical		is					D- threo-1-phenyl-2-decanoylamino-3-morpholino- 1-propanol 	Chemical				NULL		0	NULL	NULL	NULL	gw60_science_274_5294_1855_s_69	8943189	For example, the addition of precursor gangliosides, precursor sphingosine, bacterial sphingomyelinase (which generates ceramide at the plasma membrane), D- threo-1-phenyl-2-decanoylamino-3-morpholino- 1-propanol (PDMP) (which inhibits further incorporation of ceramide into glycolipids), or D- erythro-2-( N-myristoylamino)-1-phenyl-1-propanol (D-MAPP) (which inhibits ceramide metabolism through ceramidase) results in accumulation of ceramide ranging from three to eight times the concentrations in unstimulated cells ( 19).	transcription
71344	9	336173	7	NULL	NULL	NULL	NULL	D-MAPP	Chemical		results in					ceramide	Chemical	accumulation of			NULL	unstimulated cells	NULL	NULL	NULL	NULL	gw60_science_274_5294_1855_s_69	8943189	For example, the addition of precursor gangliosides, precursor sphingosine, bacterial sphingomyelinase (which generates ceramide at the plasma membrane), D- threo-1-phenyl-2-decanoylamino-3-morpholino- 1-propanol (PDMP) (which inhibits further incorporation of ceramide into glycolipids), or D- erythro-2-( N-myristoylamino)-1-phenyl-1-propanol (D-MAPP) (which inhibits ceramide metabolism through ceramidase) results in accumulation of ceramide ranging from three to eight times the concentrations in unstimulated cells ( 19).	transcription
71345	10	336173	7	NULL	NULL	0	NULL	D-MAPP	Chemical		inhibit					ceramide metabolism	Process				NULL		0	NULL	NULL	NULL	gw60_science_274_5294_1855_s_69	8943189	For example, the addition of precursor gangliosides, precursor sphingosine, bacterial sphingomyelinase (which generates ceramide at the plasma membrane), D- threo-1-phenyl-2-decanoylamino-3-morpholino- 1-propanol (PDMP) (which inhibits further incorporation of ceramide into glycolipids), or D- erythro-2-( N-myristoylamino)-1-phenyl-1-propanol (D-MAPP) (which inhibits ceramide metabolism through ceramidase) results in accumulation of ceramide ranging from three to eight times the concentrations in unstimulated cells ( 19).	transcription
71346	11	336173	7	NULL	NULL	0	NULL	statement 10	Process		occur through					ceramidase	GP				NULL		0	NULL	NULL	NULL	gw60_science_274_5294_1855_s_69	8943189	For example, the addition of precursor gangliosides, precursor sphingosine, bacterial sphingomyelinase (which generates ceramide at the plasma membrane), D- threo-1-phenyl-2-decanoylamino-3-morpholino- 1-propanol (PDMP) (which inhibits further incorporation of ceramide into glycolipids), or D- erythro-2-( N-myristoylamino)-1-phenyl-1-propanol (D-MAPP) (which inhibits ceramide metabolism through ceramidase) results in accumulation of ceramide ranging from three to eight times the concentrations in unstimulated cells ( 19).	transcription
71347	12	336173	7	NULL	NULL	0	NULL	D-MAPP	Chemical		is					D- erythro-2-( N-myristoylamino)-1-phenyl-1-propanol	Chemical				NULL		0	NULL	NULL	NULL	gw60_science_274_5294_1855_s_69	8943189	For example, the addition of precursor gangliosides, precursor sphingosine, bacterial sphingomyelinase (which generates ceramide at the plasma membrane), D- threo-1-phenyl-2-decanoylamino-3-morpholino- 1-propanol (PDMP) (which inhibits further incorporation of ceramide into glycolipids), or D- erythro-2-( N-myristoylamino)-1-phenyl-1-propanol (D-MAPP) (which inhibits ceramide metabolism through ceramidase) results in accumulation of ceramide ranging from three to eight times the concentrations in unstimulated cells ( 19).	transcription
67210	1	336174	5	NULL	NULL	0	NULL	apoptosis	Process		induced through					Fas	GP	stimulation of			NULL		0	NULL	NULL	NULL	gw60_pnas_94_14_7292_s_9	9207084	Sphingosine-based ceramides have been strongly implicated in the process of apoptosis induced (among other methods) through stimulation of the Fas ( 1-8) and tumor necrosis factor (TNF) receptors ( 7,  9-11), by UV ( 3,  7,  12) and x-ray irradiation ( 12,  13), or through treatment with certain chemotherapy drugs (refs.	transcription
67211	2	336174	5	NULL	NULL	0	NULL	apoptosis	Process		induced through					TNF receptor	GP	stimulation of			NULL		0	NULL	NULL	NULL	gw60_pnas_94_14_7292_s_9	9207084	Sphingosine-based ceramides have been strongly implicated in the process of apoptosis induced (among other methods) through stimulation of the Fas ( 1-8) and tumor necrosis factor (TNF) receptors ( 7,  9-11), by UV ( 3,  7,  12) and x-ray irradiation ( 12,  13), or through treatment with certain chemotherapy drugs (refs.	transcription
67212	3	336174	5	NULL	NULL	0	NULL	apoptosis	Process		induced by					UV					NULL		0	NULL	NULL	NULL	gw60_pnas_94_14_7292_s_9	9207084	Sphingosine-based ceramides have been strongly implicated in the process of apoptosis induced (among other methods) through stimulation of the Fas ( 1-8) and tumor necrosis factor (TNF) receptors ( 7,  9-11), by UV ( 3,  7,  12) and x-ray irradiation ( 12,  13), or through treatment with certain chemotherapy drugs (refs.	transcription
67213	4	336174	5	NULL	NULL	0	NULL	apoptosis	Process		induced by					x-ray		irradiation of			NULL		0	NULL	NULL	NULL	gw60_pnas_94_14_7292_s_9	9207084	Sphingosine-based ceramides have been strongly implicated in the process of apoptosis induced (among other methods) through stimulation of the Fas ( 1-8) and tumor necrosis factor (TNF) receptors ( 7,  9-11), by UV ( 3,  7,  12) and x-ray irradiation ( 12,  13), or through treatment with certain chemotherapy drugs (refs.	transcription
67214	5	336174	5	NULL	NULL	0	NULL	apoptosis	Process		induced through					chemotherapy drugs	Chemical	treatment with			NULL		0	NULL	NULL	NULL	gw60_pnas_94_14_7292_s_9	9207084	Sphingosine-based ceramides have been strongly implicated in the process of apoptosis induced (among other methods) through stimulation of the Fas ( 1-8) and tumor necrosis factor (TNF) receptors ( 7,  9-11), by UV ( 3,  7,  12) and x-ray irradiation ( 12,  13), or through treatment with certain chemotherapy drugs (refs.	transcription
67215	6	336174	5	NULL	NULL	0	NULL	sphingosine-based ceramides	Chemical		implicated in		strongly			statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_94_14_7292_s_9	9207084	Sphingosine-based ceramides have been strongly implicated in the process of apoptosis induced (among other methods) through stimulation of the Fas ( 1-8) and tumor necrosis factor (TNF) receptors ( 7,  9-11), by UV ( 3,  7,  12) and x-ray irradiation ( 12,  13), or through treatment with certain chemotherapy drugs (refs.	transcription
67216	7	336174	5	NULL	NULL	0	NULL	sphingosine-based ceramides	Chemical		implicated in		strongly			statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_94_14_7292_s_9	9207084	Sphingosine-based ceramides have been strongly implicated in the process of apoptosis induced (among other methods) through stimulation of the Fas ( 1-8) and tumor necrosis factor (TNF) receptors ( 7,  9-11), by UV ( 3,  7,  12) and x-ray irradiation ( 12,  13), or through treatment with certain chemotherapy drugs (refs.	transcription
67217	8	336174	5	NULL	NULL	0	NULL	Sphingosine-based ceramides	Chemical		implicated in		strongly			statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_94_14_7292_s_9	9207084	Sphingosine-based ceramides have been strongly implicated in the process of apoptosis induced (among other methods) through stimulation of the Fas ( 1-8) and tumor necrosis factor (TNF) receptors ( 7,  9-11), by UV ( 3,  7,  12) and x-ray irradiation ( 12,  13), or through treatment with certain chemotherapy drugs (refs.	transcription
67218	9	336174	5	NULL	NULL	0	NULL	Sphingosine-based ceramides	Chemical		implicated in		strongly			statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_94_14_7292_s_9	9207084	Sphingosine-based ceramides have been strongly implicated in the process of apoptosis induced (among other methods) through stimulation of the Fas ( 1-8) and tumor necrosis factor (TNF) receptors ( 7,  9-11), by UV ( 3,  7,  12) and x-ray irradiation ( 12,  13), or through treatment with certain chemotherapy drugs (refs.	transcription
67219	10	336174	5	NULL	NULL	0	NULL	sphingosine-based ceramides	Chemical		implicated in		strongly			statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_94_14_7292_s_9	9207084	Sphingosine-based ceramides have been strongly implicated in the process of apoptosis induced (among other methods) through stimulation of the Fas ( 1-8) and tumor necrosis factor (TNF) receptors ( 7,  9-11), by UV ( 3,  7,  12) and x-ray irradiation ( 12,  13), or through treatment with certain chemotherapy drugs (refs.	transcription
71348	1	336174	7	NULL	NULL	0	NULL	Sphingosine-based ceramides	Chemical		is implicated in		strongly			apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_94_14_7292_s_9	9207084	Sphingosine-based ceramides have been strongly implicated in the process of apoptosis induced (among other methods) through stimulation of the Fas ( 1-8) and tumor necrosis factor (TNF) receptors ( 7,  9-11), by UV ( 3,  7,  12) and x-ray irradiation ( 12,  13), or through treatment with certain chemotherapy drugs (refs.	transcription
71349	2	336174	7	NULL	NULL	NULL	NULL	Fas	GP	stimulation of	induce					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_94_14_7292_s_9	9207084	Sphingosine-based ceramides have been strongly implicated in the process of apoptosis induced (among other methods) through stimulation of the Fas ( 1-8) and tumor necrosis factor (TNF) receptors ( 7,  9-11), by UV ( 3,  7,  12) and x-ray irradiation ( 12,  13), or through treatment with certain chemotherapy drugs (refs.	transcription
71350	3	336174	7	NULL	NULL	0	NULL	TNF receptor	GP	stimulation of	induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_94_14_7292_s_9	9207084	Sphingosine-based ceramides have been strongly implicated in the process of apoptosis induced (among other methods) through stimulation of the Fas ( 1-8) and tumor necrosis factor (TNF) receptors ( 7,  9-11), by UV ( 3,  7,  12) and x-ray irradiation ( 12,  13), or through treatment with certain chemotherapy drugs (refs.	transcription
71351	4	336174	7	NULL	NULL	0	NULL	UV			induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_94_14_7292_s_9	9207084	Sphingosine-based ceramides have been strongly implicated in the process of apoptosis induced (among other methods) through stimulation of the Fas ( 1-8) and tumor necrosis factor (TNF) receptors ( 7,  9-11), by UV ( 3,  7,  12) and x-ray irradiation ( 12,  13), or through treatment with certain chemotherapy drugs (refs.	transcription
71352	5	336174	7	NULL	NULL	0	NULL	x-ray irradiation			induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_94_14_7292_s_9	9207084	Sphingosine-based ceramides have been strongly implicated in the process of apoptosis induced (among other methods) through stimulation of the Fas ( 1-8) and tumor necrosis factor (TNF) receptors ( 7,  9-11), by UV ( 3,  7,  12) and x-ray irradiation ( 12,  13), or through treatment with certain chemotherapy drugs (refs.	transcription
71353	6	336174	7	NULL	NULL	0	NULL	chemotherapy drugs	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_94_14_7292_s_9	9207084	Sphingosine-based ceramides have been strongly implicated in the process of apoptosis induced (among other methods) through stimulation of the Fas ( 1-8) and tumor necrosis factor (TNF) receptors ( 7,  9-11), by UV ( 3,  7,  12) and x-ray irradiation ( 12,  13), or through treatment with certain chemotherapy drugs (refs.	transcription
67220	1	336175	5	NULL	NULL	0	NULL	apoptosis	Process		induced by					Fas	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_94_14_7292_s_95	9207084	Thus, the use of a direct MS-based assay, which is highly selective and sensitive, clearly demonstrated that  in vivo generation of sphingosine-based ceramides does not occur during Fas-induced apoptosis, contrary to the many published reports mentioned above.	transcription
67221	2	336175	5	NULL	NULL	0	NULL	sphingosine-based ceramides	Chemical	in vivo generation of	does not occur during					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_94_14_7292_s_95	9207084	Thus, the use of a direct MS-based assay, which is highly selective and sensitive, clearly demonstrated that  in vivo generation of sphingosine-based ceramides does not occur during Fas-induced apoptosis, contrary to the many published reports mentioned above.	transcription
71354	1	336175	7	NULL	NULL	0	NULL	Fas	GP		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_94_14_7292_s_95	9207084	Thus, the use of a direct MS-based assay, which is highly selective and sensitive, clearly demonstrated that  in vivo generation of sphingosine-based ceramides does not occur during Fas-induced apoptosis, contrary to the many published reports mentioned above.	transcription
71355	2	336175	7	NULL	NULL	0	NULL	sphingosine-based ceramides 	Chemical	in vivo generation of	does not occur					statement 1	Process	during			NULL		0	NULL	NULL	NULL	gw60_pnas_94_14_7292_s_95	9207084	Thus, the use of a direct MS-based assay, which is highly selective and sensitive, clearly demonstrated that  in vivo generation of sphingosine-based ceramides does not occur during Fas-induced apoptosis, contrary to the many published reports mentioned above.	transcription
67222	1	336176	5	NULL	NULL	0	NULL	TAM-67	GP		is a deletion mutant of					c-Jun	GP		NH2-terminus		NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_5	9415703	Dominant-negative blockade of normal c-Jun activity by transfection with the TAM-67 c-Jun NH2-terminal deletion mutant abolished the lethal actions of ceramide but was without effect on those of sphingosine, indicating that ceramide-related apoptosis is directly dependent on activation of c-Jun, whereas sphingosine-induced cell death proceeds via an unrelated downstream mechanism.	transcription
67223	2	336176	5	NULL	NULL	0	NULL	statement 1	Process	transfection with	blocks		dominant-negative			c-Jun	GP	normal activity of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_5	9415703	Dominant-negative blockade of normal c-Jun activity by transfection with the TAM-67 c-Jun NH2-terminal deletion mutant abolished the lethal actions of ceramide but was without effect on those of sphingosine, indicating that ceramide-related apoptosis is directly dependent on activation of c-Jun, whereas sphingosine-induced cell death proceeds via an unrelated downstream mechanism.	transcription
67224	3	336176	5	NULL	NULL	0	NULL	statement 2	Process		abolishes					ceramide	Chemical	lethal actions of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_5	9415703	Dominant-negative blockade of normal c-Jun activity by transfection with the TAM-67 c-Jun NH2-terminal deletion mutant abolished the lethal actions of ceramide but was without effect on those of sphingosine, indicating that ceramide-related apoptosis is directly dependent on activation of c-Jun, whereas sphingosine-induced cell death proceeds via an unrelated downstream mechanism.	transcription
67225	4	336176	5	NULL	NULL	0	NULL	statement 2	Process		does not effect					sphingosine	Chemical	lethal actions of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_5	9415703	Dominant-negative blockade of normal c-Jun activity by transfection with the TAM-67 c-Jun NH2-terminal deletion mutant abolished the lethal actions of ceramide but was without effect on those of sphingosine, indicating that ceramide-related apoptosis is directly dependent on activation of c-Jun, whereas sphingosine-induced cell death proceeds via an unrelated downstream mechanism.	transcription
67226	5	336176	5	NULL	NULL	0	NULL	apoptosis	Process		is related to					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_5	9415703	Dominant-negative blockade of normal c-Jun activity by transfection with the TAM-67 c-Jun NH2-terminal deletion mutant abolished the lethal actions of ceramide but was without effect on those of sphingosine, indicating that ceramide-related apoptosis is directly dependent on activation of c-Jun, whereas sphingosine-induced cell death proceeds via an unrelated downstream mechanism.	transcription
67227	6	336176	5	NULL	NULL	0	NULL	statement 5	Process		is dependent on		directly			c-Jun	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_5	9415703	Dominant-negative blockade of normal c-Jun activity by transfection with the TAM-67 c-Jun NH2-terminal deletion mutant abolished the lethal actions of ceramide but was without effect on those of sphingosine, indicating that ceramide-related apoptosis is directly dependent on activation of c-Jun, whereas sphingosine-induced cell death proceeds via an unrelated downstream mechanism.	transcription
67228	7	336176	5	NULL	NULL	0	NULL	cell death	Process		induced by					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_5	9415703	Dominant-negative blockade of normal c-Jun activity by transfection with the TAM-67 c-Jun NH2-terminal deletion mutant abolished the lethal actions of ceramide but was without effect on those of sphingosine, indicating that ceramide-related apoptosis is directly dependent on activation of c-Jun, whereas sphingosine-induced cell death proceeds via an unrelated downstream mechanism.	transcription
67229	8	336176	5	NULL	NULL	0	NULL	statement 7	Process		proceeds via					unrelated downstream mechanism					NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_5	9415703	Dominant-negative blockade of normal c-Jun activity by transfection with the TAM-67 c-Jun NH2-terminal deletion mutant abolished the lethal actions of ceramide but was without effect on those of sphingosine, indicating that ceramide-related apoptosis is directly dependent on activation of c-Jun, whereas sphingosine-induced cell death proceeds via an unrelated downstream mechanism.	transcription
71356	1	336176	7	NULL	NULL	0	NULL	TAM-67 c-Jun	GP	deletion mutant	abolish			NH2-terminal		ceramide	Chemical	lethal actions of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_5	9415703	Dominant-negative blockade of normal c-Jun activity by transfection with the TAM-67 c-Jun NH2-terminal deletion mutant abolished the lethal actions of ceramide but was without effect on those of sphingosine, indicating that ceramide-related apoptosis is directly dependent on activation of c-Jun, whereas sphingosine-induced cell death proceeds via an unrelated downstream mechanism.	transcription
71357	2	336176	7	NULL	NULL	0	NULL	TAM-67 c-Jun 	GP	deletion mutant	does not effect			NH2-terminal		sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_5	9415703	Dominant-negative blockade of normal c-Jun activity by transfection with the TAM-67 c-Jun NH2-terminal deletion mutant abolished the lethal actions of ceramide but was without effect on those of sphingosine, indicating that ceramide-related apoptosis is directly dependent on activation of c-Jun, whereas sphingosine-induced cell death proceeds via an unrelated downstream mechanism.	transcription
71358	3	336176	7	NULL	NULL	NULL	NULL	ceramide	Chemical		related to					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_5	9415703	Dominant-negative blockade of normal c-Jun activity by transfection with the TAM-67 c-Jun NH2-terminal deletion mutant abolished the lethal actions of ceramide but was without effect on those of sphingosine, indicating that ceramide-related apoptosis is directly dependent on activation of c-Jun, whereas sphingosine-induced cell death proceeds via an unrelated downstream mechanism.	transcription
71359	4	336176	7	NULL	NULL	0	NULL	statement3	Process		depends on		directly			c-Jun	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_5	9415703	Dominant-negative blockade of normal c-Jun activity by transfection with the TAM-67 c-Jun NH2-terminal deletion mutant abolished the lethal actions of ceramide but was without effect on those of sphingosine, indicating that ceramide-related apoptosis is directly dependent on activation of c-Jun, whereas sphingosine-induced cell death proceeds via an unrelated downstream mechanism.	transcription
71360	5	336176	7	NULL	NULL	0	NULL	sphingosine	Chemical		induce					cell death	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_5	9415703	Dominant-negative blockade of normal c-Jun activity by transfection with the TAM-67 c-Jun NH2-terminal deletion mutant abolished the lethal actions of ceramide but was without effect on those of sphingosine, indicating that ceramide-related apoptosis is directly dependent on activation of c-Jun, whereas sphingosine-induced cell death proceeds via an unrelated downstream mechanism.	transcription
71361	6	336176	7	NULL	NULL	0	NULL	statement 5	Process		proceed via					 unrelated downstream mechanism	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_5	9415703	Dominant-negative blockade of normal c-Jun activity by transfection with the TAM-67 c-Jun NH2-terminal deletion mutant abolished the lethal actions of ceramide but was without effect on those of sphingosine, indicating that ceramide-related apoptosis is directly dependent on activation of c-Jun, whereas sphingosine-induced cell death proceeds via an unrelated downstream mechanism.	transcription
67230	1	336177	5	NULL	NULL	0	NULL	apoptosis	Process		induced by					Fas	GP				NULL	Type II Cells	0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_280	10747891	Proposed Role of Sphingosine and Ceramide in Fas-induced Apoptosis of Type II Cells-- Consistent with other studies on inhibition of Fas-induced apoptosis by Bcl-2 or Bcl-xL in type II cells ( 2,  55,  67,  87-89), we found that Bcl-xL inhibited Fas-induced apoptosis in Jurkat cells, albeit to a lesser extent than its effect on ceramide- and sphingosine-induced apoptosis.	transcription
67231	2	336177	5	NULL	NULL	0	NULL	sphingosine	Chemical		plays a role in		potentially			statement 1	Process				NULL	Type II Cells	0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_280	10747891	Proposed Role of Sphingosine and Ceramide in Fas-induced Apoptosis of Type II Cells-- Consistent with other studies on inhibition of Fas-induced apoptosis by Bcl-2 or Bcl-xL in type II cells ( 2,  55,  67,  87-89), we found that Bcl-xL inhibited Fas-induced apoptosis in Jurkat cells, albeit to a lesser extent than its effect on ceramide- and sphingosine-induced apoptosis.	transcription
67232	3	336177	5	NULL	NULL	0	NULL	ceramide	Chemical		plays a role in		potentially			statement 1	Process				NULL	Type II Cells	0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_280	10747891	Proposed Role of Sphingosine and Ceramide in Fas-induced Apoptosis of Type II Cells-- Consistent with other studies on inhibition of Fas-induced apoptosis by Bcl-2 or Bcl-xL in type II cells ( 2,  55,  67,  87-89), we found that Bcl-xL inhibited Fas-induced apoptosis in Jurkat cells, albeit to a lesser extent than its effect on ceramide- and sphingosine-induced apoptosis.	transcription
67233	4	336177	5	NULL	NULL	0	NULL	Bcl-2	GP		inhibits					statement 1	Process				NULL	Type II Cells	0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_280	10747891	Proposed Role of Sphingosine and Ceramide in Fas-induced Apoptosis of Type II Cells-- Consistent with other studies on inhibition of Fas-induced apoptosis by Bcl-2 or Bcl-xL in type II cells ( 2,  55,  67,  87-89), we found that Bcl-xL inhibited Fas-induced apoptosis in Jurkat cells, albeit to a lesser extent than its effect on ceramide- and sphingosine-induced apoptosis.	transcription
67234	5	336177	5	NULL	NULL	0	NULL	Bcl-xL	GP		inhibits					statement 1	Process				NULL	Type II Cells	0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_280	10747891	Proposed Role of Sphingosine and Ceramide in Fas-induced Apoptosis of Type II Cells-- Consistent with other studies on inhibition of Fas-induced apoptosis by Bcl-2 or Bcl-xL in type II cells ( 2,  55,  67,  87-89), we found that Bcl-xL inhibited Fas-induced apoptosis in Jurkat cells, albeit to a lesser extent than its effect on ceramide- and sphingosine-induced apoptosis.	transcription
67235	6	336177	5	NULL	NULL	0	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_280	10747891	Proposed Role of Sphingosine and Ceramide in Fas-induced Apoptosis of Type II Cells-- Consistent with other studies on inhibition of Fas-induced apoptosis by Bcl-2 or Bcl-xL in type II cells ( 2,  55,  67,  87-89), we found that Bcl-xL inhibited Fas-induced apoptosis in Jurkat cells, albeit to a lesser extent than its effect on ceramide- and sphingosine-induced apoptosis.	transcription
67236	7	336177	5	NULL	NULL	0	NULL	apoptosis	Process		induced by					Fas	GP				NULL	Jurkat cells	0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_280	10747891	Proposed Role of Sphingosine and Ceramide in Fas-induced Apoptosis of Type II Cells-- Consistent with other studies on inhibition of Fas-induced apoptosis by Bcl-2 or Bcl-xL in type II cells ( 2,  55,  67,  87-89), we found that Bcl-xL inhibited Fas-induced apoptosis in Jurkat cells, albeit to a lesser extent than its effect on ceramide- and sphingosine-induced apoptosis.	transcription
67237	8	336177	5	NULL	NULL	0	NULL	Bcl-xL	GP		inhibits					statement 7	Process				NULL	Jurkat cells	0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_280	10747891	Proposed Role of Sphingosine and Ceramide in Fas-induced Apoptosis of Type II Cells-- Consistent with other studies on inhibition of Fas-induced apoptosis by Bcl-2 or Bcl-xL in type II cells ( 2,  55,  67,  87-89), we found that Bcl-xL inhibited Fas-induced apoptosis in Jurkat cells, albeit to a lesser extent than its effect on ceramide- and sphingosine-induced apoptosis.	transcription
67238	9	336177	5	NULL	NULL	0	NULL	apoptosis	Process		induced by					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_280	10747891	Proposed Role of Sphingosine and Ceramide in Fas-induced Apoptosis of Type II Cells-- Consistent with other studies on inhibition of Fas-induced apoptosis by Bcl-2 or Bcl-xL in type II cells ( 2,  55,  67,  87-89), we found that Bcl-xL inhibited Fas-induced apoptosis in Jurkat cells, albeit to a lesser extent than its effect on ceramide- and sphingosine-induced apoptosis.	transcription
67239	10	336177	5	NULL	NULL	0	NULL	apoptosis	Process		induced by					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_280	10747891	Proposed Role of Sphingosine and Ceramide in Fas-induced Apoptosis of Type II Cells-- Consistent with other studies on inhibition of Fas-induced apoptosis by Bcl-2 or Bcl-xL in type II cells ( 2,  55,  67,  87-89), we found that Bcl-xL inhibited Fas-induced apoptosis in Jurkat cells, albeit to a lesser extent than its effect on ceramide- and sphingosine-induced apoptosis.	transcription
67240	11	336177	5	NULL	NULL	0	NULL	Bcl-xL	GP		inhibits					statement 9	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_280	10747891	Proposed Role of Sphingosine and Ceramide in Fas-induced Apoptosis of Type II Cells-- Consistent with other studies on inhibition of Fas-induced apoptosis by Bcl-2 or Bcl-xL in type II cells ( 2,  55,  67,  87-89), we found that Bcl-xL inhibited Fas-induced apoptosis in Jurkat cells, albeit to a lesser extent than its effect on ceramide- and sphingosine-induced apoptosis.	transcription
67241	12	336177	5	NULL	NULL	0	NULL	Bcl-xL	GP		inhibits					statement 10	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_280	10747891	Proposed Role of Sphingosine and Ceramide in Fas-induced Apoptosis of Type II Cells-- Consistent with other studies on inhibition of Fas-induced apoptosis by Bcl-2 or Bcl-xL in type II cells ( 2,  55,  67,  87-89), we found that Bcl-xL inhibited Fas-induced apoptosis in Jurkat cells, albeit to a lesser extent than its effect on ceramide- and sphingosine-induced apoptosis.	transcription
67242	13	336177	5	NULL	NULL	0	NULL	statement 8	Process		lesser extent than					statement 11	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_280	10747891	Proposed Role of Sphingosine and Ceramide in Fas-induced Apoptosis of Type II Cells-- Consistent with other studies on inhibition of Fas-induced apoptosis by Bcl-2 or Bcl-xL in type II cells ( 2,  55,  67,  87-89), we found that Bcl-xL inhibited Fas-induced apoptosis in Jurkat cells, albeit to a lesser extent than its effect on ceramide- and sphingosine-induced apoptosis.	transcription
67243	14	336177	5	NULL	NULL	0	NULL	statement 8	Process		lesser extent than					statement 12	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_280	10747891	Proposed Role of Sphingosine and Ceramide in Fas-induced Apoptosis of Type II Cells-- Consistent with other studies on inhibition of Fas-induced apoptosis by Bcl-2 or Bcl-xL in type II cells ( 2,  55,  67,  87-89), we found that Bcl-xL inhibited Fas-induced apoptosis in Jurkat cells, albeit to a lesser extent than its effect on ceramide- and sphingosine-induced apoptosis.	transcription
71362	1	336177	7	NULL	NULL	0	NULL	Fas	GP		induce					apoptosis	Process				NULL	Jurkat cells	0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_280	10747891	Proposed Role of Sphingosine and Ceramide in Fas-induced Apoptosis of Type II Cells-- Consistent with other studies on inhibition of Fas-induced apoptosis by Bcl-2 or Bcl-xL in type II cells ( 2,  55,  67,  87-89), we found that Bcl-xL inhibited Fas-induced apoptosis in Jurkat cells, albeit to a lesser extent than its effect on ceramide- and sphingosine-induced apoptosis.	transcription
71363	2	336177	7	NULL	NULL	0	NULL	Bcl-xL	GP		inhibit					statement 1	Process				NULL	Jurkat cells	0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_280	10747891	Proposed Role of Sphingosine and Ceramide in Fas-induced Apoptosis of Type II Cells-- Consistent with other studies on inhibition of Fas-induced apoptosis by Bcl-2 or Bcl-xL in type II cells ( 2,  55,  67,  87-89), we found that Bcl-xL inhibited Fas-induced apoptosis in Jurkat cells, albeit to a lesser extent than its effect on ceramide- and sphingosine-induced apoptosis.	transcription
71364	3	336177	7	NULL	NULL	0	NULL	ceramide	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_280	10747891	Proposed Role of Sphingosine and Ceramide in Fas-induced Apoptosis of Type II Cells-- Consistent with other studies on inhibition of Fas-induced apoptosis by Bcl-2 or Bcl-xL in type II cells ( 2,  55,  67,  87-89), we found that Bcl-xL inhibited Fas-induced apoptosis in Jurkat cells, albeit to a lesser extent than its effect on ceramide- and sphingosine-induced apoptosis.	transcription
71365	4	336177	7	NULL	NULL	0	NULL	sphingosine	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_280	10747891	Proposed Role of Sphingosine and Ceramide in Fas-induced Apoptosis of Type II Cells-- Consistent with other studies on inhibition of Fas-induced apoptosis by Bcl-2 or Bcl-xL in type II cells ( 2,  55,  67,  87-89), we found that Bcl-xL inhibited Fas-induced apoptosis in Jurkat cells, albeit to a lesser extent than its effect on ceramide- and sphingosine-induced apoptosis.	transcription
71366	5	336177	7	NULL	NULL	0	NULL	Bcl-xL	GP		inhibit					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_280	10747891	Proposed Role of Sphingosine and Ceramide in Fas-induced Apoptosis of Type II Cells-- Consistent with other studies on inhibition of Fas-induced apoptosis by Bcl-2 or Bcl-xL in type II cells ( 2,  55,  67,  87-89), we found that Bcl-xL inhibited Fas-induced apoptosis in Jurkat cells, albeit to a lesser extent than its effect on ceramide- and sphingosine-induced apoptosis.	transcription
71367	6	336177	7	NULL	NULL	0	NULL	Bcl-xL	GP		inhibit					statement 4					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_280	10747891	Proposed Role of Sphingosine and Ceramide in Fas-induced Apoptosis of Type II Cells-- Consistent with other studies on inhibition of Fas-induced apoptosis by Bcl-2 or Bcl-xL in type II cells ( 2,  55,  67,  87-89), we found that Bcl-xL inhibited Fas-induced apoptosis in Jurkat cells, albeit to a lesser extent than its effect on ceramide- and sphingosine-induced apoptosis.	transcription
71368	7	336177	7	NULL	NULL	0	NULL	statement 2	Process	inhibition of	is lesser than					statement 5	Process	inhibition of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_280	10747891	Proposed Role of Sphingosine and Ceramide in Fas-induced Apoptosis of Type II Cells-- Consistent with other studies on inhibition of Fas-induced apoptosis by Bcl-2 or Bcl-xL in type II cells ( 2,  55,  67,  87-89), we found that Bcl-xL inhibited Fas-induced apoptosis in Jurkat cells, albeit to a lesser extent than its effect on ceramide- and sphingosine-induced apoptosis.	transcription
71369	8	336177	7	NULL	NULL	0	NULL	statement 2	Process	inhibition of	is lesser than					statement 6	Process	inhibition of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_280	10747891	Proposed Role of Sphingosine and Ceramide in Fas-induced Apoptosis of Type II Cells-- Consistent with other studies on inhibition of Fas-induced apoptosis by Bcl-2 or Bcl-xL in type II cells ( 2,  55,  67,  87-89), we found that Bcl-xL inhibited Fas-induced apoptosis in Jurkat cells, albeit to a lesser extent than its effect on ceramide- and sphingosine-induced apoptosis.	transcription
71370	9	336177	7	NULL	NULL	NULL	NULL	Fas	GP		induce					apoptosis	Process				NULL	type II cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_280	10747891	Proposed Role of Sphingosine and Ceramide in Fas-induced Apoptosis of Type II Cells-- Consistent with other studies on inhibition of Fas-induced apoptosis by Bcl-2 or Bcl-xL in type II cells ( 2,  55,  67,  87-89), we found that Bcl-xL inhibited Fas-induced apoptosis in Jurkat cells, albeit to a lesser extent than its effect on ceramide- and sphingosine-induced apoptosis.	transcription
71371	10	336177	7	NULL	NULL	0	NULL	Bcl-2	GP		inhibit					statement 9	Process				NULL	type II cells	0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_280	10747891	Proposed Role of Sphingosine and Ceramide in Fas-induced Apoptosis of Type II Cells-- Consistent with other studies on inhibition of Fas-induced apoptosis by Bcl-2 or Bcl-xL in type II cells ( 2,  55,  67,  87-89), we found that Bcl-xL inhibited Fas-induced apoptosis in Jurkat cells, albeit to a lesser extent than its effect on ceramide- and sphingosine-induced apoptosis.	transcription
71372	11	336177	7	NULL	NULL	NULL	NULL	Bcl-xL	GP		inhibit					statement 9	Process				NULL	type II cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_280	10747891	Proposed Role of Sphingosine and Ceramide in Fas-induced Apoptosis of Type II Cells-- Consistent with other studies on inhibition of Fas-induced apoptosis by Bcl-2 or Bcl-xL in type II cells ( 2,  55,  67,  87-89), we found that Bcl-xL inhibited Fas-induced apoptosis in Jurkat cells, albeit to a lesser extent than its effect on ceramide- and sphingosine-induced apoptosis.	transcription
67244	1	336178	5	NULL	NULL	0	NULL	fumonisin B	Chemical		is a type of					mycotoxin	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8137_s_157	9525917	Similarly, treatment of the COS-7 cells with 5-10 muM fumonisin B, a mycotoxin that inhibits ceramide synthase and thereby blocks the acylation of sphingosine and sphinganine to form ceramide, for 10 min or with 1 unit/ml sphingomyelinase from  Bacillus cereus for 30 min also caused a stimulation of this ~68-kDa kinase which was of even greater magnitude than was observed with exogenously added sphingosine.	transcription
67245	2	336178	5	NULL	NULL	0	NULL	fumonisin B	Chemical		inhibits					ceramide syhthase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8137_s_157	9525917	Similarly, treatment of the COS-7 cells with 5-10 muM fumonisin B, a mycotoxin that inhibits ceramide synthase and thereby blocks the acylation of sphingosine and sphinganine to form ceramide, for 10 min or with 1 unit/ml sphingomyelinase from  Bacillus cereus for 30 min also caused a stimulation of this ~68-kDa kinase which was of even greater magnitude than was observed with exogenously added sphingosine.	transcription
67246	3	336178	5	NULL	NULL	0	NULL	sphingosine	Chemical	acylation of	leads to					ceramide	Chemical	formation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8137_s_157	9525917	Similarly, treatment of the COS-7 cells with 5-10 muM fumonisin B, a mycotoxin that inhibits ceramide synthase and thereby blocks the acylation of sphingosine and sphinganine to form ceramide, for 10 min or with 1 unit/ml sphingomyelinase from  Bacillus cereus for 30 min also caused a stimulation of this ~68-kDa kinase which was of even greater magnitude than was observed with exogenously added sphingosine.	transcription
67247	4	336178	5	NULL	NULL	0	NULL	sphinganine	Chemical	acylation of	leads to					ceramide	Chemical	formation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8137_s_157	9525917	Similarly, treatment of the COS-7 cells with 5-10 muM fumonisin B, a mycotoxin that inhibits ceramide synthase and thereby blocks the acylation of sphingosine and sphinganine to form ceramide, for 10 min or with 1 unit/ml sphingomyelinase from  Bacillus cereus for 30 min also caused a stimulation of this ~68-kDa kinase which was of even greater magnitude than was observed with exogenously added sphingosine.	transcription
67248	5	336178	5	NULL	NULL	0	NULL	statement 2	Process		blocks					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8137_s_157	9525917	Similarly, treatment of the COS-7 cells with 5-10 muM fumonisin B, a mycotoxin that inhibits ceramide synthase and thereby blocks the acylation of sphingosine and sphinganine to form ceramide, for 10 min or with 1 unit/ml sphingomyelinase from  Bacillus cereus for 30 min also caused a stimulation of this ~68-kDa kinase which was of even greater magnitude than was observed with exogenously added sphingosine.	transcription
67249	6	336178	5	NULL	NULL	0	NULL	statement 2	Process		blocks					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8137_s_157	9525917	Similarly, treatment of the COS-7 cells with 5-10 muM fumonisin B, a mycotoxin that inhibits ceramide synthase and thereby blocks the acylation of sphingosine and sphinganine to form ceramide, for 10 min or with 1 unit/ml sphingomyelinase from  Bacillus cereus for 30 min also caused a stimulation of this ~68-kDa kinase which was of even greater magnitude than was observed with exogenously added sphingosine.	transcription
67250	7	336178	5	NULL	NULL	0	NULL	COS-7 cells	Cell		is treated with					fumonisin B	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8137_s_157	9525917	Similarly, treatment of the COS-7 cells with 5-10 muM fumonisin B, a mycotoxin that inhibits ceramide synthase and thereby blocks the acylation of sphingosine and sphinganine to form ceramide, for 10 min or with 1 unit/ml sphingomyelinase from  Bacillus cereus for 30 min also caused a stimulation of this ~68-kDa kinase which was of even greater magnitude than was observed with exogenously added sphingosine.	transcription
67251	8	336178	5	NULL	NULL	0	NULL	COS-7 cells	Cell		is treated with					sphingomyelinase	GP	Bacillus cereus			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8137_s_157	9525917	Similarly, treatment of the COS-7 cells with 5-10 muM fumonisin B, a mycotoxin that inhibits ceramide synthase and thereby blocks the acylation of sphingosine and sphinganine to form ceramide, for 10 min or with 1 unit/ml sphingomyelinase from  Bacillus cereus for 30 min also caused a stimulation of this ~68-kDa kinase which was of even greater magnitude than was observed with exogenously added sphingosine.	transcription
67252	9	336178	5	NULL	NULL	0	NULL	statement 7	Process		stimulates					~68-kDa kinase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8137_s_157	9525917	Similarly, treatment of the COS-7 cells with 5-10 muM fumonisin B, a mycotoxin that inhibits ceramide synthase and thereby blocks the acylation of sphingosine and sphinganine to form ceramide, for 10 min or with 1 unit/ml sphingomyelinase from  Bacillus cereus for 30 min also caused a stimulation of this ~68-kDa kinase which was of even greater magnitude than was observed with exogenously added sphingosine.	transcription
67253	10	336178	5	NULL	NULL	0	NULL	statement 8	Process		stimulates					~68-kDa kinase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8137_s_157	9525917	Similarly, treatment of the COS-7 cells with 5-10 muM fumonisin B, a mycotoxin that inhibits ceramide synthase and thereby blocks the acylation of sphingosine and sphinganine to form ceramide, for 10 min or with 1 unit/ml sphingomyelinase from  Bacillus cereus for 30 min also caused a stimulation of this ~68-kDa kinase which was of even greater magnitude than was observed with exogenously added sphingosine.	transcription
67254	11	336178	5	NULL	NULL	0	NULL	COS-7 cells	Cell		is treated with					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8137_s_157	9525917	Similarly, treatment of the COS-7 cells with 5-10 muM fumonisin B, a mycotoxin that inhibits ceramide synthase and thereby blocks the acylation of sphingosine and sphinganine to form ceramide, for 10 min or with 1 unit/ml sphingomyelinase from  Bacillus cereus for 30 min also caused a stimulation of this ~68-kDa kinase which was of even greater magnitude than was observed with exogenously added sphingosine.	transcription
67255	12	336178	5	NULL	NULL	0	NULL	statement 11	Process		stimulates					~68-kDa kinase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8137_s_157	9525917	Similarly, treatment of the COS-7 cells with 5-10 muM fumonisin B, a mycotoxin that inhibits ceramide synthase and thereby blocks the acylation of sphingosine and sphinganine to form ceramide, for 10 min or with 1 unit/ml sphingomyelinase from  Bacillus cereus for 30 min also caused a stimulation of this ~68-kDa kinase which was of even greater magnitude than was observed with exogenously added sphingosine.	transcription
67256	13	336178	5	NULL	NULL	0	NULL	statement 9	Process		greater magnitude than					statement 12	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8137_s_157	9525917	Similarly, treatment of the COS-7 cells with 5-10 muM fumonisin B, a mycotoxin that inhibits ceramide synthase and thereby blocks the acylation of sphingosine and sphinganine to form ceramide, for 10 min or with 1 unit/ml sphingomyelinase from  Bacillus cereus for 30 min also caused a stimulation of this ~68-kDa kinase which was of even greater magnitude than was observed with exogenously added sphingosine.	transcription
67257	14	336178	5	NULL	NULL	0	NULL	statement 10	Process		greater magnitude than					statement 12					NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8137_s_157	9525917	Similarly, treatment of the COS-7 cells with 5-10 muM fumonisin B, a mycotoxin that inhibits ceramide synthase and thereby blocks the acylation of sphingosine and sphinganine to form ceramide, for 10 min or with 1 unit/ml sphingomyelinase from  Bacillus cereus for 30 min also caused a stimulation of this ~68-kDa kinase which was of even greater magnitude than was observed with exogenously added sphingosine.	transcription
71373	1	336178	7	NULL	NULL	0	NULL	fumonisin B	Chemical		inhibit					ceramide synthase	GP				NULL	COS-7 cells	0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8137_s_157	9525917	Similarly, treatment of the COS-7 cells with 5-10 muM fumonisin B, a mycotoxin that inhibits ceramide synthase and thereby blocks the acylation of sphingosine and sphinganine to form ceramide, for 10 min or with 1 unit/ml sphingomyelinase from  Bacillus cereus for 30 min also caused a stimulation of this ~68-kDa kinase which was of even greater magnitude than was observed with exogenously added sphingosine.	transcription
71374	2	336178	7	NULL	NULL	0	NULL	statement 1	Process		blocks 					sphingosine	Chemical	acylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8137_s_157	9525917	Similarly, treatment of the COS-7 cells with 5-10 muM fumonisin B, a mycotoxin that inhibits ceramide synthase and thereby blocks the acylation of sphingosine and sphinganine to form ceramide, for 10 min or with 1 unit/ml sphingomyelinase from  Bacillus cereus for 30 min also caused a stimulation of this ~68-kDa kinase which was of even greater magnitude than was observed with exogenously added sphingosine.	transcription
71375	3	336178	7	NULL	NULL	0	NULL	statement 1	Process		blocks					sphinganine	Chemical	acylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8137_s_157	9525917	Similarly, treatment of the COS-7 cells with 5-10 muM fumonisin B, a mycotoxin that inhibits ceramide synthase and thereby blocks the acylation of sphingosine and sphinganine to form ceramide, for 10 min or with 1 unit/ml sphingomyelinase from  Bacillus cereus for 30 min also caused a stimulation of this ~68-kDa kinase which was of even greater magnitude than was observed with exogenously added sphingosine.	transcription
71376	4	336178	7	NULL	NULL	0	NULL	sphingosine	Chemical	acylation of	forms					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8137_s_157	9525917	Similarly, treatment of the COS-7 cells with 5-10 muM fumonisin B, a mycotoxin that inhibits ceramide synthase and thereby blocks the acylation of sphingosine and sphinganine to form ceramide, for 10 min or with 1 unit/ml sphingomyelinase from  Bacillus cereus for 30 min also caused a stimulation of this ~68-kDa kinase which was of even greater magnitude than was observed with exogenously added sphingosine.	transcription
71377	5	336178	7	NULL	NULL	0	NULL	sphinganine	Chemical	acylation of	forms					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8137_s_157	9525917	Similarly, treatment of the COS-7 cells with 5-10 muM fumonisin B, a mycotoxin that inhibits ceramide synthase and thereby blocks the acylation of sphingosine and sphinganine to form ceramide, for 10 min or with 1 unit/ml sphingomyelinase from  Bacillus cereus for 30 min also caused a stimulation of this ~68-kDa kinase which was of even greater magnitude than was observed with exogenously added sphingosine.	transcription
71378	6	336178	7	NULL	NULL	0	NULL	fumonisin B	Chemical		is a type of					mycotoxin	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_14_8137_s_157	9525917	Similarly, treatment of the COS-7 cells with 5-10 muM fumonisin B, a mycotoxin that inhibits ceramide synthase and thereby blocks the acylation of sphingosine and sphinganine to form ceramide, for 10 min or with 1 unit/ml sphingomyelinase from  Bacillus cereus for 30 min also caused a stimulation of this ~68-kDa kinase which was of even greater magnitude than was observed with exogenously added sphingosine.	transcription
67258	1	336179	5	NULL	NULL	0	NULL	ceramide	Chemical		induces		directly			apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
67259	2	336179	5	NULL	NULL	0	NULL	ceramide	Chemical	elevations of	induced by					agonist	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
67260	3	336179	5	NULL	NULL	0	NULL	statement 2	Process		precede					apoptosis	Process	biochemical manifestations of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
67261	4	336179	5	NULL	NULL	0	NULL	statement 2	Process		precede					apoptosis	Process	morphological manifestations of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
67262	5	336179	5	NULL	NULL	0	NULL	ceramide	Chemical	natural	elevates					ceramide	Chemical	cellular			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
67263	6	336179	5	NULL	NULL	0	NULL	stress	Process		effects					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
67264	7	336179	5	NULL	NULL	0	NULL	statement 5	Process		mimics					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
67265	8	336179	5	NULL	NULL	0	NULL	ceramide analogs	Chemical		elevates					ceramide	Chemical	cellular			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
67266	9	336179	5	NULL	NULL	0	NULL	statement 8	Process		mimics					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
67267	10	336179	5	NULL	NULL	0	NULL	SMases	GP		elevates					ceramide	Chemical	cellular			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
67268	11	336179	5	NULL	NULL	0	NULL	statement 10	Process		mimics					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
67269	12	336179	5	NULL	NULL	0	NULL	pharmacological agents	Chemical		interfere with					ceramide metabolism enzymes	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
67270	13	336179	5	NULL	NULL	0	NULL	statement 12	Process		elevates					ceramide	Chemical	cellular			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
67271	14	336179	5	NULL	NULL	0	NULL	D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol	Chemical		is an inhibitor of					glucosylceramide synthase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
67272	15	336179	5	NULL	NULL	0	NULL	N-oleoylethanolamine	Chemical		is an inhibitor of					ceramidase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
67273	16	336179	5	NULL	NULL	0	NULL	D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol	Chemical		is a type of					pharmacological agent	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
67274	17	336179	5	NULL	NULL	0	NULL	N-oleoylethanolamine			is a type of					pharmacological agents	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
67275	18	336179	5	NULL	NULL	0	NULL	statement 13	Process		enhance					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
67276	19	336179	5	NULL	NULL	0	NULL	fumonisin B1	Chemical		is an inhibitor of					ceramide syhthase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
67277	20	336179	5	NULL	NULL	0	NULL	statement 19	Process		reduce					ceramide	Chemical	generation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
67278	21	336179	5	NULL	NULL	0	NULL	statement 20	Process		prevent					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
67279	22	336179	5	NULL	NULL	0	NULL	lipids	Chemical		fail to signal		consistently			apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
67280	23	336179	5	NULL	NULL	0	NULL	sphingolipid metabolites	Chemical		fail to signal		consistently			apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
67281	24	336179	5	NULL	NULL	0	NULL	sphingosine	Chemical		does not fail to signal					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71379	1	336179	7	NULL	NULL	0	NULL	 ceramide	Chemical		is involved in		directly			apoptosis	Process	induction of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71380	2	336179	7	NULL	NULL	0	NULL	agonist	Chemical		induce					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71381	3	336179	7	NULL	NULL	0	NULL	apoptosis	Process	biochemical manifestations of	precede					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71382	4	336179	7	NULL	NULL	0	NULL	apoptosis	Process	morphological manifestations of	precede					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71383	5	336179	7	NULL	NULL	0	NULL	natural ceramide	Chemical		elevates					cellular ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71384	6	336179	7	NULL	NULL	0	NULL	 ceramide analogs	Chemical		elevates					cellular ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71385	7	336179	7	NULL	NULL	0	NULL	 SMases	GP	exogenous	elevates					cellular ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71386	8	336179	7	NULL	NULL	0	NULL	statement 5	Process		mimic					apoptosis	Process	effects of stress on			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71387	9	336179	7	NULL	NULL	0	NULL	statement 6	Process		mimic					apoptosis	Process	effects of stress on			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71388	10	336179	7	NULL	NULL	0	NULL	statement 7	Process		mimic					apoptosis	Process	effects of stress on			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71389	11	336179	7	NULL	NULL	0	NULL	D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol 	Chemical		inhibit					glucosylceramide synthase	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71390	12	336179	7	NULL	NULL	0	NULL	D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol 	Chemical		interferes with					ceramide metabolism	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71391	13	336179	7	NULL	NULL	0	NULL	D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol 	Chemical		elevate					cellular ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71392	14	336179	7	NULL	NULL	0	NULL	N-oleoylethanolamine	Chemical		inhibit					ceramidase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71393	15	336179	7	NULL	NULL	0	NULL	N-oleoylethanolamine	Chemical		interferes with					ceramide metabolism	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71394	16	336179	7	NULL	NULL	0	NULL	N-oleoylethanolamine	Chemical		elevate					cellular ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71395	17	336179	7	NULL	NULL	0	NULL	D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol	Chemical		enhance		uniformly			apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71396	18	336179	7	NULL	NULL	0	NULL	N-oleoylethanolamine	Chemical		enhance		uniformly			apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71397	19	336179	7	NULL	NULL	0	NULL	fumonisin B1	Chemical		inhibit					ceramide synthase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71398	20	336179	7	NULL	NULL	0	NULL	fumonisin B1	Chemical		prevent					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71399	21	336179	7	NULL	NULL	0	NULL	fumonisin B1	Chemical		reduce					ceramide	Chemical	generation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71400	22	336179	7	NULL	NULL	0	NULL	sphingolipid metabolites	Chemical		fail to		consistently			apoptosis	Process	signal			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71401	23	336179	7	NULL	NULL	0	NULL	sphingosine	Chemical		signals					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71402	24	336179	7	NULL	NULL	0	NULL	statement 3	Process		support					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71403	25	336179	7	NULL	NULL	0	NULL	statement 4	Process		support					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71404	26	336179	7	NULL	NULL	0	NULL	statement 8	Process		support					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71405	27	336179	7	NULL	NULL	0	NULL	statement 9	Process		support					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71406	28	336179	7	NULL	NULL	0	NULL	statement 10	Process		support					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71407	29	336179	7	NULL	NULL	0	NULL	statement 17	Process		support					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71408	30	336179	7	NULL	NULL	0	NULL	statement 18	Process		support					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71409	31	336179	7	NULL	NULL	0	NULL	statement 20	Process		support					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
71410	32	336179	7	NULL	NULL	0	NULL	statement 22	Process		support					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_442_s_15	11031259	Evidence that ceramide is involved directly in the induction of apoptosis is summarized as follows: (i) agonist-induced ceramide elevations precede biochemical and morphological manifestations of apoptosis ( 4-7); (ii) elevation of cellular ceramide levels using natural ceramide ( 8-10), ceramide analogs, or exogenous SMases mimic the effects of stress on apoptosis ( 11-16); (iii) pharmacological agents which interfere with enzymes of ceramide metabolism and elevate cellular ceramide, such as the glucosylceramide synthase inhibitor D-threo-1-phenyl-decanoylamino-3-morpholino-1-propanol or the ceramidase inhibitor  N-oleoylethanolamine, uniformly enhance apoptosis ( 17-19), whereas agents that reduce ceramide generation, such as the ceramide synthase inhibitor fumonisin B1, prevent apoptosis ( 10,  20,  21); and (iv) other lipids, including other sphingolipid metabolites (except perhaps sphingosine), fail to consistently signal apoptosis ( 12,  13,  16).	transcription
67282	1	336180	5	NULL	NULL	0	NULL	sphingosine	Chemical		induces					c-Jun	GP	expression of			NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_135	12135749	Here we demonstrated that (i) sphingosine (as well as ceramide) induced c-jun expression, (ii) sphingosine-induced c-jun expression was stimulated by H-89, a PKA inhibitor, whereas C2-ceramide-induced c-jun expression was not affected by H-89, (iii) sphingosine-induced c-jun expression was only slightly affected by PKC inhibitors, whereas C2-ceramide-induced c-jun expression was strongly inhibited by PKC inhibitors.	transcription
67283	2	336180	5	NULL	NULL	0	NULL	ceramide	Chemical		induces					c-Jun	GP	expression of			NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_135	12135749	Here we demonstrated that (i) sphingosine (as well as ceramide) induced c-jun expression, (ii) sphingosine-induced c-jun expression was stimulated by H-89, a PKA inhibitor, whereas C2-ceramide-induced c-jun expression was not affected by H-89, (iii) sphingosine-induced c-jun expression was only slightly affected by PKC inhibitors, whereas C2-ceramide-induced c-jun expression was strongly inhibited by PKC inhibitors.	transcription
67284	3	336180	5	NULL	NULL	0	NULL	H-89	Chemical		is an inhibitor of					PKA	GP				NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_135	12135749	Here we demonstrated that (i) sphingosine (as well as ceramide) induced c-jun expression, (ii) sphingosine-induced c-jun expression was stimulated by H-89, a PKA inhibitor, whereas C2-ceramide-induced c-jun expression was not affected by H-89, (iii) sphingosine-induced c-jun expression was only slightly affected by PKC inhibitors, whereas C2-ceramide-induced c-jun expression was strongly inhibited by PKC inhibitors.	transcription
67285	4	336180	5	NULL	NULL	0	NULL	H-89	Chemical		stimulates					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_135	12135749	Here we demonstrated that (i) sphingosine (as well as ceramide) induced c-jun expression, (ii) sphingosine-induced c-jun expression was stimulated by H-89, a PKA inhibitor, whereas C2-ceramide-induced c-jun expression was not affected by H-89, (iii) sphingosine-induced c-jun expression was only slightly affected by PKC inhibitors, whereas C2-ceramide-induced c-jun expression was strongly inhibited by PKC inhibitors.	transcription
67286	5	336180	5	NULL	NULL	0	NULL	C2-ceramide	Chemical		induces					c-Jun	GP	expression of			NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_135	12135749	Here we demonstrated that (i) sphingosine (as well as ceramide) induced c-jun expression, (ii) sphingosine-induced c-jun expression was stimulated by H-89, a PKA inhibitor, whereas C2-ceramide-induced c-jun expression was not affected by H-89, (iii) sphingosine-induced c-jun expression was only slightly affected by PKC inhibitors, whereas C2-ceramide-induced c-jun expression was strongly inhibited by PKC inhibitors.	transcription
67287	6	336180	5	NULL	NULL	0	NULL	H-89	Chemical		does not affect					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_135	12135749	Here we demonstrated that (i) sphingosine (as well as ceramide) induced c-jun expression, (ii) sphingosine-induced c-jun expression was stimulated by H-89, a PKA inhibitor, whereas C2-ceramide-induced c-jun expression was not affected by H-89, (iii) sphingosine-induced c-jun expression was only slightly affected by PKC inhibitors, whereas C2-ceramide-induced c-jun expression was strongly inhibited by PKC inhibitors.	transcription
67288	7	336180	5	NULL	NULL	0	NULL	PKC inhibitors	Chemical		affects		slightly			statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_135	12135749	Here we demonstrated that (i) sphingosine (as well as ceramide) induced c-jun expression, (ii) sphingosine-induced c-jun expression was stimulated by H-89, a PKA inhibitor, whereas C2-ceramide-induced c-jun expression was not affected by H-89, (iii) sphingosine-induced c-jun expression was only slightly affected by PKC inhibitors, whereas C2-ceramide-induced c-jun expression was strongly inhibited by PKC inhibitors.	transcription
67289	8	336180	5	NULL	NULL	0	NULL	PKC inhibitors	Chemical		inhibits		strongly			statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_135	12135749	Here we demonstrated that (i) sphingosine (as well as ceramide) induced c-jun expression, (ii) sphingosine-induced c-jun expression was stimulated by H-89, a PKA inhibitor, whereas C2-ceramide-induced c-jun expression was not affected by H-89, (iii) sphingosine-induced c-jun expression was only slightly affected by PKC inhibitors, whereas C2-ceramide-induced c-jun expression was strongly inhibited by PKC inhibitors.	transcription
71411	1	336180	7	NULL	NULL	0	NULL	sphingosine	Chemical		induce					c-jun	GP	expression of			NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_135	12135749	Here we demonstrated that (i) sphingosine (as well as ceramide) induced c-jun expression, (ii) sphingosine-induced c-jun expression was stimulated by H-89, a PKA inhibitor, whereas C2-ceramide-induced c-jun expression was not affected by H-89, (iii) sphingosine-induced c-jun expression was only slightly affected by PKC inhibitors, whereas C2-ceramide-induced c-jun expression was strongly inhibited by PKC inhibitors.	transcription
71412	2	336180	7	NULL	NULL	0	NULL	ceramide	Chemical		induce					c-jun	GP	expression of			NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_135	12135749	Here we demonstrated that (i) sphingosine (as well as ceramide) induced c-jun expression, (ii) sphingosine-induced c-jun expression was stimulated by H-89, a PKA inhibitor, whereas C2-ceramide-induced c-jun expression was not affected by H-89, (iii) sphingosine-induced c-jun expression was only slightly affected by PKC inhibitors, whereas C2-ceramide-induced c-jun expression was strongly inhibited by PKC inhibitors.	transcription
71413	3	336180	7	NULL	NULL	0	NULL	H-89	Chemical		stimulate					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_135	12135749	Here we demonstrated that (i) sphingosine (as well as ceramide) induced c-jun expression, (ii) sphingosine-induced c-jun expression was stimulated by H-89, a PKA inhibitor, whereas C2-ceramide-induced c-jun expression was not affected by H-89, (iii) sphingosine-induced c-jun expression was only slightly affected by PKC inhibitors, whereas C2-ceramide-induced c-jun expression was strongly inhibited by PKC inhibitors.	transcription
71414	4	336180	7	NULL	NULL	0	NULL	H-89	Chemical		is a type of					PKA inhibitor	Chemical				NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_135	12135749	Here we demonstrated that (i) sphingosine (as well as ceramide) induced c-jun expression, (ii) sphingosine-induced c-jun expression was stimulated by H-89, a PKA inhibitor, whereas C2-ceramide-induced c-jun expression was not affected by H-89, (iii) sphingosine-induced c-jun expression was only slightly affected by PKC inhibitors, whereas C2-ceramide-induced c-jun expression was strongly inhibited by PKC inhibitors.	transcription
71415	5	336180	7	NULL	NULL	0	NULL	C2-ceramide	Chemical		induce					c-jun	GP	expression of			NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_135	12135749	Here we demonstrated that (i) sphingosine (as well as ceramide) induced c-jun expression, (ii) sphingosine-induced c-jun expression was stimulated by H-89, a PKA inhibitor, whereas C2-ceramide-induced c-jun expression was not affected by H-89, (iii) sphingosine-induced c-jun expression was only slightly affected by PKC inhibitors, whereas C2-ceramide-induced c-jun expression was strongly inhibited by PKC inhibitors.	transcription
71416	6	336180	7	NULL	NULL	0	NULL	H-89	Chemical		does not affect					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_135	12135749	Here we demonstrated that (i) sphingosine (as well as ceramide) induced c-jun expression, (ii) sphingosine-induced c-jun expression was stimulated by H-89, a PKA inhibitor, whereas C2-ceramide-induced c-jun expression was not affected by H-89, (iii) sphingosine-induced c-jun expression was only slightly affected by PKC inhibitors, whereas C2-ceramide-induced c-jun expression was strongly inhibited by PKC inhibitors.	transcription
71417	7	336180	7	NULL	NULL	0	NULL	PKC inhibitors	Chemical		affect		slightly			statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_135	12135749	Here we demonstrated that (i) sphingosine (as well as ceramide) induced c-jun expression, (ii) sphingosine-induced c-jun expression was stimulated by H-89, a PKA inhibitor, whereas C2-ceramide-induced c-jun expression was not affected by H-89, (iii) sphingosine-induced c-jun expression was only slightly affected by PKC inhibitors, whereas C2-ceramide-induced c-jun expression was strongly inhibited by PKC inhibitors.	transcription
71418	8	336180	7	NULL	NULL	0	NULL	PKC inhibitors	Chemical		inhibit		strongly			statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_febslett_524_1_103_s_135	12135749	Here we demonstrated that (i) sphingosine (as well as ceramide) induced c-jun expression, (ii) sphingosine-induced c-jun expression was stimulated by H-89, a PKA inhibitor, whereas C2-ceramide-induced c-jun expression was not affected by H-89, (iii) sphingosine-induced c-jun expression was only slightly affected by PKC inhibitors, whereas C2-ceramide-induced c-jun expression was strongly inhibited by PKC inhibitors.	transcription
67290	1	336181	5	NULL	NULL	0	NULL	apoptosis	Process		induced by					Fas	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_58	10747891	Early Transient Increases in Ceramide and Sphingosine during Fas-induced Apoptosis Precede Executioner Caspases Activation and Cell Death and Are Followed by a Sustained Accumulation of Ceramide-- As previously reported ( 10,  14,  20,  21), we found that treatment of Jurkat cells with 50 ng/ml anti-Fas antibody resulted in acute changes in ceramide levels within 30 min from a basal level of ~10 pmol/nmol total phospholipids (Fig.  1 A).	transcription
67291	2	336181	5	NULL	NULL	0	NULL	ceramide	Chemical	early;;transient increase of	occurs during					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_58	10747891	Early Transient Increases in Ceramide and Sphingosine during Fas-induced Apoptosis Precede Executioner Caspases Activation and Cell Death and Are Followed by a Sustained Accumulation of Ceramide-- As previously reported ( 10,  14,  20,  21), we found that treatment of Jurkat cells with 50 ng/ml anti-Fas antibody resulted in acute changes in ceramide levels within 30 min from a basal level of ~10 pmol/nmol total phospholipids (Fig.  1 A).	transcription
67292	3	336181	5	NULL	NULL	0	NULL	sphingosine	Chemical	early;;transient increase of	occurs during					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_58	10747891	Early Transient Increases in Ceramide and Sphingosine during Fas-induced Apoptosis Precede Executioner Caspases Activation and Cell Death and Are Followed by a Sustained Accumulation of Ceramide-- As previously reported ( 10,  14,  20,  21), we found that treatment of Jurkat cells with 50 ng/ml anti-Fas antibody resulted in acute changes in ceramide levels within 30 min from a basal level of ~10 pmol/nmol total phospholipids (Fig.  1 A).	transcription
67293	4	336181	5	NULL	NULL	0	NULL	statement 2	Process		precede					executioner caspases	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_58	10747891	Early Transient Increases in Ceramide and Sphingosine during Fas-induced Apoptosis Precede Executioner Caspases Activation and Cell Death and Are Followed by a Sustained Accumulation of Ceramide-- As previously reported ( 10,  14,  20,  21), we found that treatment of Jurkat cells with 50 ng/ml anti-Fas antibody resulted in acute changes in ceramide levels within 30 min from a basal level of ~10 pmol/nmol total phospholipids (Fig.  1 A).	transcription
67294	5	336181	5	NULL	NULL	0	NULL	statement 2	Process		precede					cell death	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_58	10747891	Early Transient Increases in Ceramide and Sphingosine during Fas-induced Apoptosis Precede Executioner Caspases Activation and Cell Death and Are Followed by a Sustained Accumulation of Ceramide-- As previously reported ( 10,  14,  20,  21), we found that treatment of Jurkat cells with 50 ng/ml anti-Fas antibody resulted in acute changes in ceramide levels within 30 min from a basal level of ~10 pmol/nmol total phospholipids (Fig.  1 A).	transcription
67295	6	336181	5	NULL	NULL	0	NULL	statement 3	Process		precede					executioner caspases	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_58	10747891	Early Transient Increases in Ceramide and Sphingosine during Fas-induced Apoptosis Precede Executioner Caspases Activation and Cell Death and Are Followed by a Sustained Accumulation of Ceramide-- As previously reported ( 10,  14,  20,  21), we found that treatment of Jurkat cells with 50 ng/ml anti-Fas antibody resulted in acute changes in ceramide levels within 30 min from a basal level of ~10 pmol/nmol total phospholipids (Fig.  1 A).	transcription
67296	7	336181	5	NULL	NULL	0	NULL	statement 3	Process		precede					cell death	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_58	10747891	Early Transient Increases in Ceramide and Sphingosine during Fas-induced Apoptosis Precede Executioner Caspases Activation and Cell Death and Are Followed by a Sustained Accumulation of Ceramide-- As previously reported ( 10,  14,  20,  21), we found that treatment of Jurkat cells with 50 ng/ml anti-Fas antibody resulted in acute changes in ceramide levels within 30 min from a basal level of ~10 pmol/nmol total phospholipids (Fig.  1 A).	transcription
67297	8	336181	5	NULL	NULL	0	NULL	statement 2	Process		followed by					ceramide	Chemical	sustained accumulation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_58	10747891	Early Transient Increases in Ceramide and Sphingosine during Fas-induced Apoptosis Precede Executioner Caspases Activation and Cell Death and Are Followed by a Sustained Accumulation of Ceramide-- As previously reported ( 10,  14,  20,  21), we found that treatment of Jurkat cells with 50 ng/ml anti-Fas antibody resulted in acute changes in ceramide levels within 30 min from a basal level of ~10 pmol/nmol total phospholipids (Fig.  1 A).	transcription
67298	9	336181	5	NULL	NULL	0	NULL	statement 3	Process		followed by					ceramide	Chemical	sustained accumulation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_58	10747891	Early Transient Increases in Ceramide and Sphingosine during Fas-induced Apoptosis Precede Executioner Caspases Activation and Cell Death and Are Followed by a Sustained Accumulation of Ceramide-- As previously reported ( 10,  14,  20,  21), we found that treatment of Jurkat cells with 50 ng/ml anti-Fas antibody resulted in acute changes in ceramide levels within 30 min from a basal level of ~10 pmol/nmol total phospholipids (Fig.  1 A).	transcription
67299	10	336181	5	NULL	NULL	NULL	NULL	anti-Fas antibody	GP	treatment	results in					ceramide	Chemical	acute change of;;level of			NULL	Jurkat cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_58	10747891	Early Transient Increases in Ceramide and Sphingosine during Fas-induced Apoptosis Precede Executioner Caspases Activation and Cell Death and Are Followed by a Sustained Accumulation of Ceramide-- As previously reported ( 10,  14,  20,  21), we found that treatment of Jurkat cells with 50 ng/ml anti-Fas antibody resulted in acute changes in ceramide levels within 30 min from a basal level of ~10 pmol/nmol total phospholipids (Fig.  1 A).	transcription
71419	1	336181	7	NULL	NULL	0	NULL	Fas	GP		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_58	10747891	Early Transient Increases in Ceramide and Sphingosine during Fas-induced Apoptosis Precede Executioner Caspases Activation and Cell Death and Are Followed by a Sustained Accumulation of Ceramide-- As previously reported ( 10,  14,  20,  21), we found that treatment of Jurkat cells with 50 ng/ml anti-Fas antibody resulted in acute changes in ceramide levels within 30 min from a basal level of ~10 pmol/nmol total phospholipids (Fig.  1 A).	transcription
71420	2	336181	7	NULL	NULL	0	NULL	ceramide	Chemical	Transient Increases in	occur during					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_58	10747891	Early Transient Increases in Ceramide and Sphingosine during Fas-induced Apoptosis Precede Executioner Caspases Activation and Cell Death and Are Followed by a Sustained Accumulation of Ceramide-- As previously reported ( 10,  14,  20,  21), we found that treatment of Jurkat cells with 50 ng/ml anti-Fas antibody resulted in acute changes in ceramide levels within 30 min from a basal level of ~10 pmol/nmol total phospholipids (Fig.  1 A).	transcription
71421	3	336181	7	NULL	NULL	0	NULL	sphingosine	Chemical	Transient Increases in	occur during					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_58	10747891	Early Transient Increases in Ceramide and Sphingosine during Fas-induced Apoptosis Precede Executioner Caspases Activation and Cell Death and Are Followed by a Sustained Accumulation of Ceramide-- As previously reported ( 10,  14,  20,  21), we found that treatment of Jurkat cells with 50 ng/ml anti-Fas antibody resulted in acute changes in ceramide levels within 30 min from a basal level of ~10 pmol/nmol total phospholipids (Fig.  1 A).	transcription
71422	4	336181	7	NULL	NULL	0	NULL	statement 2	Process		precede					executioner caspases	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_58	10747891	Early Transient Increases in Ceramide and Sphingosine during Fas-induced Apoptosis Precede Executioner Caspases Activation and Cell Death and Are Followed by a Sustained Accumulation of Ceramide-- As previously reported ( 10,  14,  20,  21), we found that treatment of Jurkat cells with 50 ng/ml anti-Fas antibody resulted in acute changes in ceramide levels within 30 min from a basal level of ~10 pmol/nmol total phospholipids (Fig.  1 A).	transcription
71423	5	336181	7	NULL	NULL	0	NULL	statement 2	Process		precede					cell death	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_58	10747891	Early Transient Increases in Ceramide and Sphingosine during Fas-induced Apoptosis Precede Executioner Caspases Activation and Cell Death and Are Followed by a Sustained Accumulation of Ceramide-- As previously reported ( 10,  14,  20,  21), we found that treatment of Jurkat cells with 50 ng/ml anti-Fas antibody resulted in acute changes in ceramide levels within 30 min from a basal level of ~10 pmol/nmol total phospholipids (Fig.  1 A).	transcription
71424	6	336181	7	NULL	NULL	0	NULL	statement 4	Process		followed by					ceramide	Chemical	accumulation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_58	10747891	Early Transient Increases in Ceramide and Sphingosine during Fas-induced Apoptosis Precede Executioner Caspases Activation and Cell Death and Are Followed by a Sustained Accumulation of Ceramide-- As previously reported ( 10,  14,  20,  21), we found that treatment of Jurkat cells with 50 ng/ml anti-Fas antibody resulted in acute changes in ceramide levels within 30 min from a basal level of ~10 pmol/nmol total phospholipids (Fig.  1 A).	transcription
71425	7	336181	7	NULL	NULL	0	NULL	statement 5	Process		followed by					ceramide	Chemical	accumulation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_58	10747891	Early Transient Increases in Ceramide and Sphingosine during Fas-induced Apoptosis Precede Executioner Caspases Activation and Cell Death and Are Followed by a Sustained Accumulation of Ceramide-- As previously reported ( 10,  14,  20,  21), we found that treatment of Jurkat cells with 50 ng/ml anti-Fas antibody resulted in acute changes in ceramide levels within 30 min from a basal level of ~10 pmol/nmol total phospholipids (Fig.  1 A).	transcription
67300	1	336182	5	NULL	NULL	NULL	NULL	sphingosine kinase gene	GP	temporal expression patterns of;;Drosophila	affects					long chain base	Chemical	metabolism of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_18_18403_s_227	15734735	Furthermore, our results as well as recent work from the laboratory of Ruth Lehmann indicate that the temporal and tissue-specific expression patterns of additional  Drosophila genes affecting long chain base metabolism, including sphingosine kinase, ceramidase, and ceramide kinase, are similar to that of SPL ( ,  ).	transcription
67301	2	336182	5	NULL	NULL	0	NULL	sphingosine kinase gene	GP	tissue-specific expression patterns of;;Drosophila	affects					long chain base	Chemical	metabolism of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_18_18403_s_227	15734735	Furthermore, our results as well as recent work from the laboratory of Ruth Lehmann indicate that the temporal and tissue-specific expression patterns of additional  Drosophila genes affecting long chain base metabolism, including sphingosine kinase, ceramidase, and ceramide kinase, are similar to that of SPL ( ,  ).	transcription
67302	3	336182	5	NULL	NULL	0	NULL	statement 1	Process		similar to					SPL	GP	temporal expression patterns of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_18_18403_s_227	15734735	Furthermore, our results as well as recent work from the laboratory of Ruth Lehmann indicate that the temporal and tissue-specific expression patterns of additional  Drosophila genes affecting long chain base metabolism, including sphingosine kinase, ceramidase, and ceramide kinase, are similar to that of SPL ( ,  ).	transcription
67303	4	336182	5	NULL	NULL	0	NULL	statement 2	Process		similar to					SPL	GP	tissue-specific expression patterns of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_18_18403_s_227	15734735	Furthermore, our results as well as recent work from the laboratory of Ruth Lehmann indicate that the temporal and tissue-specific expression patterns of additional  Drosophila genes affecting long chain base metabolism, including sphingosine kinase, ceramidase, and ceramide kinase, are similar to that of SPL ( ,  ).	transcription
67304	5	336182	5	NULL	NULL	0	NULL	ceramidase gene	GP	temporal expression patterns of;;Drosophila	affects					long chain base	Chemical	metabolism of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_18_18403_s_227	15734735	Furthermore, our results as well as recent work from the laboratory of Ruth Lehmann indicate that the temporal and tissue-specific expression patterns of additional  Drosophila genes affecting long chain base metabolism, including sphingosine kinase, ceramidase, and ceramide kinase, are similar to that of SPL ( ,  ).	transcription
67305	6	336182	5	NULL	NULL	0	NULL	ceramidase gene	GP	tissue-specific expression patterns of;;Drosophila	affects					long chain base	Chemical	metabolism of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_18_18403_s_227	15734735	Furthermore, our results as well as recent work from the laboratory of Ruth Lehmann indicate that the temporal and tissue-specific expression patterns of additional  Drosophila genes affecting long chain base metabolism, including sphingosine kinase, ceramidase, and ceramide kinase, are similar to that of SPL ( ,  ).	transcription
67306	7	336182	5	NULL	NULL	0	NULL	statement 5	Process		similar to					SPL	GP	temporal expression patterns of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_18_18403_s_227	15734735	Furthermore, our results as well as recent work from the laboratory of Ruth Lehmann indicate that the temporal and tissue-specific expression patterns of additional  Drosophila genes affecting long chain base metabolism, including sphingosine kinase, ceramidase, and ceramide kinase, are similar to that of SPL ( ,  ).	transcription
67307	8	336182	5	NULL	NULL	0	NULL	statement 6	Process		similar to					SPL	GP	tissue-specific expression patterns of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_18_18403_s_227	15734735	Furthermore, our results as well as recent work from the laboratory of Ruth Lehmann indicate that the temporal and tissue-specific expression patterns of additional  Drosophila genes affecting long chain base metabolism, including sphingosine kinase, ceramidase, and ceramide kinase, are similar to that of SPL ( ,  ).	transcription
67308	9	336182	5	NULL	NULL	0	NULL	ceramide kinase gene	GP	temporal expression patterns of;;Drosophila	affects					long chain base	Chemical	metabolism of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_18_18403_s_227	15734735	Furthermore, our results as well as recent work from the laboratory of Ruth Lehmann indicate that the temporal and tissue-specific expression patterns of additional  Drosophila genes affecting long chain base metabolism, including sphingosine kinase, ceramidase, and ceramide kinase, are similar to that of SPL ( ,  ).	transcription
67309	10	336182	5	NULL	NULL	0	NULL	ceramide kinase gene	GP	tissue-specific expression patterns of;;Drosophila	affects					long chain base	Chemical	metabolism of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_18_18403_s_227	15734735	Furthermore, our results as well as recent work from the laboratory of Ruth Lehmann indicate that the temporal and tissue-specific expression patterns of additional  Drosophila genes affecting long chain base metabolism, including sphingosine kinase, ceramidase, and ceramide kinase, are similar to that of SPL ( ,  ).	transcription
67310	11	336182	5	NULL	NULL	0	NULL	statement 9	Process		similar to					SPL	GP	temporal expression patterns of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_18_18403_s_227	15734735	Furthermore, our results as well as recent work from the laboratory of Ruth Lehmann indicate that the temporal and tissue-specific expression patterns of additional  Drosophila genes affecting long chain base metabolism, including sphingosine kinase, ceramidase, and ceramide kinase, are similar to that of SPL ( ,  ).	transcription
67311	12	336182	5	NULL	NULL	0	NULL	statement 10	Process		similar to					SPL	GP	tissue-specific expression patterns of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_18_18403_s_227	15734735	Furthermore, our results as well as recent work from the laboratory of Ruth Lehmann indicate that the temporal and tissue-specific expression patterns of additional  Drosophila genes affecting long chain base metabolism, including sphingosine kinase, ceramidase, and ceramide kinase, are similar to that of SPL ( ,  ).	transcription
71426	1	336182	7	NULL	NULL	0	NULL	Drosophila genes	GP	temporal specific expression patterns of	affect					long chain base metabolism	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_18_18403_s_227	15734735	Furthermore, our results as well as recent work from the laboratory of Ruth Lehmann indicate that the temporal and tissue-specific expression patterns of additional  Drosophila genes affecting long chain base metabolism, including sphingosine kinase, ceramidase, and ceramide kinase, are similar to that of SPL ( ,  ).	transcription
71427	2	336182	7	NULL	NULL	0	NULL	Drosophila genes	GP	tissue-specific expression patterns of	affect					long chain base metabolism	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_18_18403_s_227	15734735	Furthermore, our results as well as recent work from the laboratory of Ruth Lehmann indicate that the temporal and tissue-specific expression patterns of additional  Drosophila genes affecting long chain base metabolism, including sphingosine kinase, ceramidase, and ceramide kinase, are similar to that of SPL ( ,  ).	transcription
71428	3	336182	7	NULL	NULL	0	NULL	statement 1	Process		affect					sphingosine kinase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_18_18403_s_227	15734735	Furthermore, our results as well as recent work from the laboratory of Ruth Lehmann indicate that the temporal and tissue-specific expression patterns of additional  Drosophila genes affecting long chain base metabolism, including sphingosine kinase, ceramidase, and ceramide kinase, are similar to that of SPL ( ,  ).	transcription
71429	4	336182	7	NULL	NULL	0	NULL	statement 2	Process		affect					sphingosine kinase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_18_18403_s_227	15734735	Furthermore, our results as well as recent work from the laboratory of Ruth Lehmann indicate that the temporal and tissue-specific expression patterns of additional  Drosophila genes affecting long chain base metabolism, including sphingosine kinase, ceramidase, and ceramide kinase, are similar to that of SPL ( ,  ).	transcription
71430	5	336182	7	NULL	NULL	0	NULL	statement 1	Process		affect					ceramidase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_18_18403_s_227	15734735	Furthermore, our results as well as recent work from the laboratory of Ruth Lehmann indicate that the temporal and tissue-specific expression patterns of additional  Drosophila genes affecting long chain base metabolism, including sphingosine kinase, ceramidase, and ceramide kinase, are similar to that of SPL ( ,  ).	transcription
71431	6	336182	7	NULL	NULL	0	NULL	statement 2	Process		affect					ceramidase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_18_18403_s_227	15734735	Furthermore, our results as well as recent work from the laboratory of Ruth Lehmann indicate that the temporal and tissue-specific expression patterns of additional  Drosophila genes affecting long chain base metabolism, including sphingosine kinase, ceramidase, and ceramide kinase, are similar to that of SPL ( ,  ).	transcription
71432	7	336182	7	NULL	NULL	0	NULL	statement 1	Process		affect					ceramide kinase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_18_18403_s_227	15734735	Furthermore, our results as well as recent work from the laboratory of Ruth Lehmann indicate that the temporal and tissue-specific expression patterns of additional  Drosophila genes affecting long chain base metabolism, including sphingosine kinase, ceramidase, and ceramide kinase, are similar to that of SPL ( ,  ).	transcription
71433	8	336182	7	NULL	NULL	NULL	NULL	statement 2	Process		affect					ceramide kinase	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_18_18403_s_227	15734735	Furthermore, our results as well as recent work from the laboratory of Ruth Lehmann indicate that the temporal and tissue-specific expression patterns of additional  Drosophila genes affecting long chain base metabolism, including sphingosine kinase, ceramidase, and ceramide kinase, are similar to that of SPL ( ,  ).	transcription
67312	1	336183	5	NULL	NULL	0	NULL	sphingosine	Chemical		is phosphorylated to					S1-P	Chemical				NULL		0	NULL	NULL	NULL	gw60_genetics_156_4_1519_s_227	11102354	On the other hand, S1-P, which is formed by phosphorylation of sphingosine, has been implicated in a number of important cellular functions including promotion of cell proliferation and inhibition of cell motility, tumor cell invasiveness, ceramide-mediated apoptosis, and developmental processes.	transcription
67313	2	336183	5	NULL	NULL	0	NULL	S1-P	Chemical		promotes					cell proliferation	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_156_4_1519_s_227	11102354	On the other hand, S1-P, which is formed by phosphorylation of sphingosine, has been implicated in a number of important cellular functions including promotion of cell proliferation and inhibition of cell motility, tumor cell invasiveness, ceramide-mediated apoptosis, and developmental processes.	transcription
67314	3	336183	5	NULL	NULL	0	NULL	S1-P	Chemical		inhibits					cell motility	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_156_4_1519_s_227	11102354	On the other hand, S1-P, which is formed by phosphorylation of sphingosine, has been implicated in a number of important cellular functions including promotion of cell proliferation and inhibition of cell motility, tumor cell invasiveness, ceramide-mediated apoptosis, and developmental processes.	transcription
67315	4	336183	5	NULL	NULL	0	NULL	S1-P	Chemical		inhibits					tumor cell	Cell	invasiveness of			NULL		0	NULL	NULL	NULL	gw60_genetics_156_4_1519_s_227	11102354	On the other hand, S1-P, which is formed by phosphorylation of sphingosine, has been implicated in a number of important cellular functions including promotion of cell proliferation and inhibition of cell motility, tumor cell invasiveness, ceramide-mediated apoptosis, and developmental processes.	transcription
67316	5	336183	5	NULL	NULL	0	NULL	apoptosis	Process		is mediated by					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_genetics_156_4_1519_s_227	11102354	On the other hand, S1-P, which is formed by phosphorylation of sphingosine, has been implicated in a number of important cellular functions including promotion of cell proliferation and inhibition of cell motility, tumor cell invasiveness, ceramide-mediated apoptosis, and developmental processes.	transcription
67317	6	336183	5	NULL	NULL	0	NULL	S1-P	Chemical		inhibits					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_156_4_1519_s_227	11102354	On the other hand, S1-P, which is formed by phosphorylation of sphingosine, has been implicated in a number of important cellular functions including promotion of cell proliferation and inhibition of cell motility, tumor cell invasiveness, ceramide-mediated apoptosis, and developmental processes.	transcription
67318	7	336183	5	NULL	NULL	0	NULL	S1-P	Chemical		inhibits					developmental processes	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_156_4_1519_s_227	11102354	On the other hand, S1-P, which is formed by phosphorylation of sphingosine, has been implicated in a number of important cellular functions including promotion of cell proliferation and inhibition of cell motility, tumor cell invasiveness, ceramide-mediated apoptosis, and developmental processes.	transcription
71434	1	336183	7	NULL	NULL	0	NULL	sphingosine	Chemical	phosphorylation of	forms					S1-P	Chemical				NULL		0	NULL	NULL	NULL	gw60_genetics_156_4_1519_s_227	11102354	On the other hand, S1-P, which is formed by phosphorylation of sphingosine, has been implicated in a number of important cellular functions including promotion of cell proliferation and inhibition of cell motility, tumor cell invasiveness, ceramide-mediated apoptosis, and developmental processes.	transcription
71435	2	336183	7	NULL	NULL	NULL	NULL	S1-P	Chemical		promote					cell proliferation	Process				NULL		NULL	NULL	NULL	NULL	gw60_genetics_156_4_1519_s_227	11102354	On the other hand, S1-P, which is formed by phosphorylation of sphingosine, has been implicated in a number of important cellular functions including promotion of cell proliferation and inhibition of cell motility, tumor cell invasiveness, ceramide-mediated apoptosis, and developmental processes.	transcription
71436	3	336183	7	NULL	NULL	0	NULL	S1-P	Chemical		inhibit					cell motility	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_156_4_1519_s_227	11102354	On the other hand, S1-P, which is formed by phosphorylation of sphingosine, has been implicated in a number of important cellular functions including promotion of cell proliferation and inhibition of cell motility, tumor cell invasiveness, ceramide-mediated apoptosis, and developmental processes.	transcription
71437	4	336183	7	NULL	NULL	0	NULL	S1-P	Chemical		inhibit					tumor cell invasiveness	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_156_4_1519_s_227	11102354	On the other hand, S1-P, which is formed by phosphorylation of sphingosine, has been implicated in a number of important cellular functions including promotion of cell proliferation and inhibition of cell motility, tumor cell invasiveness, ceramide-mediated apoptosis, and developmental processes.	transcription
71438	5	336183	7	NULL	NULL	0	NULL	ceramide	Chemical		mediates					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_156_4_1519_s_227	11102354	On the other hand, S1-P, which is formed by phosphorylation of sphingosine, has been implicated in a number of important cellular functions including promotion of cell proliferation and inhibition of cell motility, tumor cell invasiveness, ceramide-mediated apoptosis, and developmental processes.	transcription
71439	6	336183	7	NULL	NULL	0	NULL	S1-P	Chemical		inhibit					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_156_4_1519_s_227	11102354	On the other hand, S1-P, which is formed by phosphorylation of sphingosine, has been implicated in a number of important cellular functions including promotion of cell proliferation and inhibition of cell motility, tumor cell invasiveness, ceramide-mediated apoptosis, and developmental processes.	transcription
71440	7	336183	7	NULL	NULL	0	NULL	S1-P	Chemical		inhibit					developmental processes	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_156_4_1519_s_227	11102354	On the other hand, S1-P, which is formed by phosphorylation of sphingosine, has been implicated in a number of important cellular functions including promotion of cell proliferation and inhibition of cell motility, tumor cell invasiveness, ceramide-mediated apoptosis, and developmental processes.	transcription
67319	1	336184	5	NULL	NULL	NULL	NULL	Sphingosine 1-phosphate	GP		inhibits					caspases	GP	activation of			NULL	Jurkat T lymphocytes	NULL	NULL	NULL	NULL	gw60_genetics_156_4_1519_s_279	11102354	CUVILLIER, O., D. S. ROSENTHAL, M. E. SMULSON, and S. SPIEGEL, 1998  Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide-mediated apoptosis in Jurkat T lymphocytes.	transcription
67320	2	336184	5	NULL	NULL	0	NULL	caspases	GP		cleave					poly(ADP-ribose) polymerase	GP				NULL	Jurkat T lymphocytes	0	NULL	NULL	NULL	gw60_genetics_156_4_1519_s_279	11102354	CUVILLIER, O., D. S. ROSENTHAL, M. E. SMULSON, and S. SPIEGEL, 1998  Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide-mediated apoptosis in Jurkat T lymphocytes.	transcription
67321	3	336184	5	NULL	NULL	0	NULL	caspases	GP		cleave					lamins	GP				NULL	Jurkat T lymphocytes	0	NULL	NULL	NULL	gw60_genetics_156_4_1519_s_279	11102354	CUVILLIER, O., D. S. ROSENTHAL, M. E. SMULSON, and S. SPIEGEL, 1998  Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide-mediated apoptosis in Jurkat T lymphocytes.	transcription
67322	4	336184	5	NULL	NULL	0	NULL	apoptosis	Process		is mediated by					Fas	GP				NULL	Jurkat T lymphocytes	0	NULL	NULL	NULL	gw60_genetics_156_4_1519_s_279	11102354	CUVILLIER, O., D. S. ROSENTHAL, M. E. SMULSON, and S. SPIEGEL, 1998  Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide-mediated apoptosis in Jurkat T lymphocytes.	transcription
67323	5	336184	5	NULL	NULL	0	NULL	apoptosis	Process		is mediated by					ceramide	Chemical				NULL	Jurkat T lymphocytes	0	NULL	NULL	NULL	gw60_genetics_156_4_1519_s_279	11102354	CUVILLIER, O., D. S. ROSENTHAL, M. E. SMULSON, and S. SPIEGEL, 1998  Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide-mediated apoptosis in Jurkat T lymphocytes.	transcription
67324	6	336184	5	NULL	NULL	0	NULL	statement 2	Process		occurs during					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_156_4_1519_s_279	11102354	CUVILLIER, O., D. S. ROSENTHAL, M. E. SMULSON, and S. SPIEGEL, 1998  Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide-mediated apoptosis in Jurkat T lymphocytes.	transcription
67325	7	336184	5	NULL	NULL	0	NULL	statement 2	Process		occurs during					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_156_4_1519_s_279	11102354	CUVILLIER, O., D. S. ROSENTHAL, M. E. SMULSON, and S. SPIEGEL, 1998  Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide-mediated apoptosis in Jurkat T lymphocytes.	transcription
67326	8	336184	5	NULL	NULL	0	NULL	statement 3	Process		occurs during					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_156_4_1519_s_279	11102354	CUVILLIER, O., D. S. ROSENTHAL, M. E. SMULSON, and S. SPIEGEL, 1998  Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide-mediated apoptosis in Jurkat T lymphocytes.	transcription
67327	9	336184	5	NULL	NULL	0	NULL	statement 3	Process		occurs during					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_genetics_156_4_1519_s_279	11102354	CUVILLIER, O., D. S. ROSENTHAL, M. E. SMULSON, and S. SPIEGEL, 1998  Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide-mediated apoptosis in Jurkat T lymphocytes.	transcription
71441	1	336184	7	NULL	NULL	0	NULL	caspases	GP		cleave					poly(ADP-ribose) polymerase	GP				NULL		0	NULL	NULL	NULL	gw60_genetics_156_4_1519_s_279	11102354	CUVILLIER, O., D. S. ROSENTHAL, M. E. SMULSON, and S. SPIEGEL, 1998  Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide-mediated apoptosis in Jurkat T lymphocytes.	transcription
71442	2	336184	7	NULL	NULL	0	NULL	caspases	GP		cleave					lamins	Chemical				NULL		0	NULL	NULL	NULL	gw60_genetics_156_4_1519_s_279	11102354	CUVILLIER, O., D. S. ROSENTHAL, M. E. SMULSON, and S. SPIEGEL, 1998  Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide-mediated apoptosis in Jurkat T lymphocytes.	transcription
71444	3	336184	7	NULL	NULL	0	NULL	Fas	GP		mediates					apoptosis	Process				NULL	Jurkat T lymphocytes	0	NULL	NULL	NULL	gw60_genetics_156_4_1519_s_279	11102354	CUVILLIER, O., D. S. ROSENTHAL, M. E. SMULSON, and S. SPIEGEL, 1998  Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide-mediated apoptosis in Jurkat T lymphocytes.	transcription
71445	4	336184	7	NULL	NULL	0	NULL	ceramide	Chemical		mediates					apoptosis	Process				NULL	Jurkat T lymphocytes	0	NULL	NULL	NULL	gw60_genetics_156_4_1519_s_279	11102354	CUVILLIER, O., D. S. ROSENTHAL, M. E. SMULSON, and S. SPIEGEL, 1998  Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide-mediated apoptosis in Jurkat T lymphocytes.	transcription
71446	5	336184	7	NULL	NULL	0	NULL	Sphingosine 1-phosphate	Chemical		inhibit					caspases	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_genetics_156_4_1519_s_279	11102354	CUVILLIER, O., D. S. ROSENTHAL, M. E. SMULSON, and S. SPIEGEL, 1998  Sphingosine 1-phosphate inhibits activation of caspases that cleave poly(ADP-ribose) polymerase and lamins during Fas- and ceramide-mediated apoptosis in Jurkat T lymphocytes.	transcription
67328	1	336185	5	NULL	NULL	0	NULL	NOE	Chemical		is an inhibitor of					ceramidase	GP				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_126_1_189_s_185	10051135	The ceramidase inhibitor, NOE, which attenuated the depressant actions of TNF under constant flow and constant pressure conditions, disrupts signalling through sphingomyelin breakdown by inhibiting the conversion of ceramide to sphingosine (Sugita  et al., 1975  ), an action which appears to be specific for the SMase pathway (Coroneos  et al., 1995  ).	transcription
67329	2	336185	5	NULL	NULL	0	NULL	NOE	Chemical		attenuates					TNF	GP	depressant actions of			NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_126_1_189_s_185	10051135	The ceramidase inhibitor, NOE, which attenuated the depressant actions of TNF under constant flow and constant pressure conditions, disrupts signalling through sphingomyelin breakdown by inhibiting the conversion of ceramide to sphingosine (Sugita  et al., 1975  ), an action which appears to be specific for the SMase pathway (Coroneos  et al., 1995  ).	transcription
67330	3	336185	5	NULL	NULL	0	NULL	statement 2	Process		under conditions of					flow	Process	constant			NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_126_1_189_s_185	10051135	The ceramidase inhibitor, NOE, which attenuated the depressant actions of TNF under constant flow and constant pressure conditions, disrupts signalling through sphingomyelin breakdown by inhibiting the conversion of ceramide to sphingosine (Sugita  et al., 1975  ), an action which appears to be specific for the SMase pathway (Coroneos  et al., 1995  ).	transcription
67331	4	336185	5	NULL	NULL	NULL	NULL	statement 2	Process		under conditions of					pressure	PhysicalPhenomenon	constant			NULL		NULL	NULL	NULL	NULL	gw60_brjpharmacol_126_1_189_s_185	10051135	The ceramidase inhibitor, NOE, which attenuated the depressant actions of TNF under constant flow and constant pressure conditions, disrupts signalling through sphingomyelin breakdown by inhibiting the conversion of ceramide to sphingosine (Sugita  et al., 1975  ), an action which appears to be specific for the SMase pathway (Coroneos  et al., 1995  ).	transcription
67332	5	336185	5	NULL	NULL	0	NULL	statement 2	Process		disrupt					signalling	Process				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_126_1_189_s_185	10051135	The ceramidase inhibitor, NOE, which attenuated the depressant actions of TNF under constant flow and constant pressure conditions, disrupts signalling through sphingomyelin breakdown by inhibiting the conversion of ceramide to sphingosine (Sugita  et al., 1975  ), an action which appears to be specific for the SMase pathway (Coroneos  et al., 1995  ).	transcription
67333	6	336185	5	NULL	NULL	0	NULL	statement 5	Process		occurs through					sphingomyelin	Chemical	breakdown of			NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_126_1_189_s_185	10051135	The ceramidase inhibitor, NOE, which attenuated the depressant actions of TNF under constant flow and constant pressure conditions, disrupts signalling through sphingomyelin breakdown by inhibiting the conversion of ceramide to sphingosine (Sugita  et al., 1975  ), an action which appears to be specific for the SMase pathway (Coroneos  et al., 1995  ).	transcription
67334	7	336185	5	NULL	NULL	0	NULL	ceramide	Chemical		converted to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_126_1_189_s_185	10051135	The ceramidase inhibitor, NOE, which attenuated the depressant actions of TNF under constant flow and constant pressure conditions, disrupts signalling through sphingomyelin breakdown by inhibiting the conversion of ceramide to sphingosine (Sugita  et al., 1975  ), an action which appears to be specific for the SMase pathway (Coroneos  et al., 1995  ).	transcription
67335	8	336185	5	NULL	NULL	0	NULL	statement 2	Process		inhibits					statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_126_1_189_s_185	10051135	The ceramidase inhibitor, NOE, which attenuated the depressant actions of TNF under constant flow and constant pressure conditions, disrupts signalling through sphingomyelin breakdown by inhibiting the conversion of ceramide to sphingosine (Sugita  et al., 1975  ), an action which appears to be specific for the SMase pathway (Coroneos  et al., 1995  ).	transcription
67336	9	336185	5	NULL	NULL	0	NULL	statement 8	Process		leads to					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_126_1_189_s_185	10051135	The ceramidase inhibitor, NOE, which attenuated the depressant actions of TNF under constant flow and constant pressure conditions, disrupts signalling through sphingomyelin breakdown by inhibiting the conversion of ceramide to sphingosine (Sugita  et al., 1975  ), an action which appears to be specific for the SMase pathway (Coroneos  et al., 1995  ).	transcription
67337	10	336185	5	NULL	NULL	0	NULL	statement 7	Process		is specific to					SMase pathway	Process				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_126_1_189_s_185	10051135	The ceramidase inhibitor, NOE, which attenuated the depressant actions of TNF under constant flow and constant pressure conditions, disrupts signalling through sphingomyelin breakdown by inhibiting the conversion of ceramide to sphingosine (Sugita  et al., 1975  ), an action which appears to be specific for the SMase pathway (Coroneos  et al., 1995  ).	transcription
71447	1	336185	7	NULL	NULL	0	NULL	NOE	Chemical		attenuate					TNF	GP	depressant actions of			NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_126_1_189_s_185	10051135	The ceramidase inhibitor, NOE, which attenuated the depressant actions of TNF under constant flow and constant pressure conditions, disrupts signalling through sphingomyelin breakdown by inhibiting the conversion of ceramide to sphingosine (Sugita  et al., 1975  ), an action which appears to be specific for the SMase pathway (Coroneos  et al., 1995  ).	transcription
71448	2	336185	7	NULL	NULL	0	NULL	NOE	Chemical		inhibit					ceramidase	GP				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_126_1_189_s_185	10051135	The ceramidase inhibitor, NOE, which attenuated the depressant actions of TNF under constant flow and constant pressure conditions, disrupts signalling through sphingomyelin breakdown by inhibiting the conversion of ceramide to sphingosine (Sugita  et al., 1975  ), an action which appears to be specific for the SMase pathway (Coroneos  et al., 1995  ).	transcription
71449	3	336185	7	NULL	NULL	0	NULL	ceramide	Chemical		converted to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_126_1_189_s_185	10051135	The ceramidase inhibitor, NOE, which attenuated the depressant actions of TNF under constant flow and constant pressure conditions, disrupts signalling through sphingomyelin breakdown by inhibiting the conversion of ceramide to sphingosine (Sugita  et al., 1975  ), an action which appears to be specific for the SMase pathway (Coroneos  et al., 1995  ).	transcription
71450	4	336185	7	NULL	NULL	0	NULL	NOE	Chemical		disrupt					signaling	Process				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_126_1_189_s_185	10051135	The ceramidase inhibitor, NOE, which attenuated the depressant actions of TNF under constant flow and constant pressure conditions, disrupts signalling through sphingomyelin breakdown by inhibiting the conversion of ceramide to sphingosine (Sugita  et al., 1975  ), an action which appears to be specific for the SMase pathway (Coroneos  et al., 1995  ).	transcription
71451	5	336185	7	NULL	NULL	0	NULL	statement 4	Process		occur through					sphingomyelin	Chemical	breakdown of			NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_126_1_189_s_185	10051135	The ceramidase inhibitor, NOE, which attenuated the depressant actions of TNF under constant flow and constant pressure conditions, disrupts signalling through sphingomyelin breakdown by inhibiting the conversion of ceramide to sphingosine (Sugita  et al., 1975  ), an action which appears to be specific for the SMase pathway (Coroneos  et al., 1995  ).	transcription
71452	6	336185	7	NULL	NULL	0	NULL	statement 5	Process		occur by					statement 3	Process	inhibition of			NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_126_1_189_s_185	10051135	The ceramidase inhibitor, NOE, which attenuated the depressant actions of TNF under constant flow and constant pressure conditions, disrupts signalling through sphingomyelin breakdown by inhibiting the conversion of ceramide to sphingosine (Sugita  et al., 1975  ), an action which appears to be specific for the SMase pathway (Coroneos  et al., 1995  ).	transcription
71453	7	336185	7	NULL	NULL	0	NULL	statement 3	Process		specific for					SMase pathway	Process				NULL		0	NULL	NULL	NULL	gw60_brjpharmacol_126_1_189_s_185	10051135	The ceramidase inhibitor, NOE, which attenuated the depressant actions of TNF under constant flow and constant pressure conditions, disrupts signalling through sphingomyelin breakdown by inhibiting the conversion of ceramide to sphingosine (Sugita  et al., 1975  ), an action which appears to be specific for the SMase pathway (Coroneos  et al., 1995  ).	transcription
67338	1	336186	5	NULL	NULL	0	NULL	TNF-alpha	GP		activates					Ras	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67339	2	336186	5	NULL	NULL	0	NULL	TNF-alpha	GP		activates					PI 3-K	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67340	3	336186	5	NULL	NULL	0	NULL	TNF-alpha	GP		activates					SK	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67341	4	336186	5	NULL	NULL	0	NULL	TNF-alpha	GP		activates					Cdc42	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67342	5	336186	5	NULL	NULL	0	NULL	TNF-alpha	GP		activates					Rac	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67343	6	336186	5	NULL	NULL	0	NULL	TNF-alpha	GP		activates					Rho	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67344	7	336186	5	NULL	NULL	0	NULL	TNF-alpha	GP		activates					PAK	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67345	8	336186	5	NULL	NULL	NULL	NULL	statement 1	Process		phosphorylates					FAK	GP		tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67346	9	336186	5	NULL	NULL	NULL	NULL	statement 1	Process		phosphorylates					paxillin	GP		tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67347	10	336186	5	NULL	NULL	0	NULL	statement 2	Process		phosphorylates					FAK	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67348	11	336186	5	NULL	NULL	0	NULL	statement 2	Process		phosphorylates					paxillin	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67349	12	336186	5	NULL	NULL	0	NULL	statement 3	Process		phosphorylates					FAK	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67350	13	336186	5	NULL	NULL	0	NULL	statement 3	Process		phosphorylates					paxillin	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67351	14	336186	5	NULL	NULL	0	NULL	statement 4	Process		phosphorylates					FAK	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67352	15	336186	5	NULL	NULL	0	NULL	statement 4	Process		phosphorylates					paxillin	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67353	16	336186	5	NULL	NULL	0	NULL	statement 5	Process		phosphorylates					FAK	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67354	17	336186	5	NULL	NULL	0	NULL	statement 5	Process		phosphorylates					paxillin	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67355	18	336186	5	NULL	NULL	0	NULL	statement 6	Process		phosphorylates					FAK	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67356	19	336186	5	NULL	NULL	0	NULL	statement 6	Process		phosphorylates					paxillin	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67357	20	336186	5	NULL	NULL	0	NULL	statement 7	Process		phosphorylates					FAK	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67358	21	336186	5	NULL	NULL	0	NULL	statement 7	Process		phosphorylates					paxillin	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67359	22	336186	5	NULL	NULL	0	NULL	sphingomyelinase	GP		activates					Ras	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67360	23	336186	5	NULL	NULL	0	NULL	statement 22	Process		phosphorylates					FAK	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67361	24	336186	5	NULL	NULL	0	NULL	statement 22	Process		phosphorylates					paxillin	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67362	25	336186	5	NULL	NULL	0	NULL	sphingomyelinase	GP		activates					PI 3-K	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67363	26	336186	5	NULL	NULL	0	NULL	statement 25	Process		phosphorylates					FAK	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67364	27	336186	5	NULL	NULL	0	NULL	statement 25	Process		phosphorylates					paxillin	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67365	28	336186	5	NULL	NULL	0	NULL	sphingomyelinase	GP		activates					SK	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67366	29	336186	5	NULL	NULL	NULL	NULL	statement 28	Process		phosphorylates					FAK	GP		tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67367	30	336186	5	NULL	NULL	0	NULL	statement 28	Process		phosphorylates					paxillin	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67368	31	336186	5	NULL	NULL	0	NULL	sphingomyelinase	GP		activates					Cdc42	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67369	32	336186	5	NULL	NULL	0	NULL	statement 31	Process		phosphorylates					FAK	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67370	33	336186	5	NULL	NULL	0	NULL	statement 31	Process		phosphorylates					paxillin	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67371	34	336186	5	NULL	NULL	0	NULL	sphingomyelinase	GP		activates					Rac	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67372	35	336186	5	NULL	NULL	0	NULL	statement 34	Process		phosphorylates					FAK	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67373	36	336186	5	NULL	NULL	0	NULL	statement 34	Process		phosphorylates					paxillin	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67374	37	336186	5	NULL	NULL	0	NULL	sphingomyelinase	GP		activates					Rho	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67376	38	336186	5	NULL	NULL	0	NULL	statement 37	Process		phosphorylates					FAK	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67379	39	336186	5	NULL	NULL	0	NULL	statement 37	Process		phosphorylates					paxillin	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67380	40	336186	5	NULL	NULL	0	NULL	sphingomyelinase	GP		activates					PAK	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67381	41	336186	5	NULL	NULL	0	NULL	statement 40	Process		phosphorylates					FAK	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67382	42	336186	5	NULL	NULL	0	NULL	statement 40	Process		phosphorylates					paxillin	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67383	43	336186	5	NULL	NULL	0	NULL	C2-ceramide	Chemical		activates					Ras	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67384	44	336186	5	NULL	NULL	0	NULL	statement 43	Process		phosphorylates					FAK	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67385	45	336186	5	NULL	NULL	0	NULL	statement 43	Process		phosphorylates					paxillin	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67386	46	336186	5	NULL	NULL	0	NULL	C2-ceramide	Chemical		activates					PI 3-K	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67387	47	336186	5	NULL	NULL	0	NULL	statement 46	Process		phosphorylates					FAK	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67388	48	336186	5	NULL	NULL	0	NULL	statement 46	Process		phosphorylates					paxillin	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67389	49	336186	5	NULL	NULL	0	NULL	C2-ceramide	Chemical		activates					SK	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67390	50	336186	5	NULL	NULL	0	NULL	statement 49	Process		phosphorylates					FAK	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67391	51	336186	5	NULL	NULL	0	NULL	statement 49	Process		phosphorylates					paxillin	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67392	52	336186	5	NULL	NULL	0	NULL	C2-ceramide	Chemical		activates					Cdc42	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67393	53	336186	5	NULL	NULL	0	NULL	statement 52	Process		phosphorylates					FAK	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67394	54	336186	5	NULL	NULL	0	NULL	statement 52	Process		phosphorylates					paxillin	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67395	55	336186	5	NULL	NULL	0	NULL	C2-ceramide	Chemical		activates					Rac	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67396	56	336186	5	NULL	NULL	0	NULL	statement 55	Process		phosphorylates					FAK	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67397	57	336186	5	NULL	NULL	0	NULL	statement 55	Process		phosphorylates					paxillin	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67398	58	336186	5	NULL	NULL	0	NULL	C2-ceramide	Chemical		activates					Rho	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67399	59	336186	5	NULL	NULL	0	NULL	statement 58	Process		phosphorylates					FAK	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67400	60	336186	5	NULL	NULL	0	NULL	statement 58	Process		phosphorylates					paxillin	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67401	61	336186	5	NULL	NULL	0	NULL	C2-ceramide	Chemical		activates					PAK	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67402	62	336186	5	NULL	NULL	0	NULL	statement 61	Process		phosphorylates					FAK	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67404	63	336186	5	NULL	NULL	0	NULL	statement 61	Process		phosphorylates					paxillin	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67405	64	336186	5	NULL	NULL	0	NULL	C2-ceramide	Chemical		is a type of					cell-permeable ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67406	65	336186	5	NULL	NULL	0	NULL	SK	GP		is					sphingosine kinase	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
67407	66	336186	5	NULL	NULL	0	NULL	PAK	GP		is					p21-activated protein kinase	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
71454	1	336186	7	NULL	NULL	0	NULL	TNF-alpha	GP		activate					Ras	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
71455	2	336186	7	NULL	NULL	0	NULL	TNF-alpha	GP		activate					PI 3-K	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
71456	3	336186	7	NULL	NULL	0	NULL	TNF-alpha	GP		activate					SK	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
71457	4	336186	7	NULL	NULL	0	NULL	TNF-alpha	GP		activate					Cdc42	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
71458	5	336186	7	NULL	NULL	0	NULL	TNF-alpha	GP		activate					Rac	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
71459	6	336186	7	NULL	NULL	0	NULL	TNF-alpha	GP		activate					Rho	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
71460	7	336186	7	NULL	NULL	0	NULL	TNF-alpha	GP		activate					PAK	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
71461	8	336186	7	NULL	NULL	0	NULL	TNF-alpha	GP		phosphorylate					FAK	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
71462	9	336186	7	NULL	NULL	0	NULL	TNF-alpha	GP		phosphorylate					paxillin	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
71463	10	336186	7	NULL	NULL	0	NULL	sphingomyelinase	GP		activate					Ras	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
71464	11	336186	7	NULL	NULL	0	NULL	sphingomyelinase	GP		activate					PI 3-K	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
71465	12	336186	7	NULL	NULL	0	NULL	sphingomyelinase	GP		activate					SK	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
71466	13	336186	7	NULL	NULL	0	NULL	sphingomyelinase	GP		activate					Cdc42	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
71467	14	336186	7	NULL	NULL	0	NULL	sphingomyelinase	GP		activate					Rac	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
71468	15	336186	7	NULL	NULL	0	NULL	sphingomyelinase	GP		activate					Rho	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
71469	16	336186	7	NULL	NULL	0	NULL	sphingomyelinase	GP		activate					PAK	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
71470	17	336186	7	NULL	NULL	0	NULL	sphingomyelinase	GP		phosphorylate					FAK	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
71471	18	336186	7	NULL	NULL	0	NULL	sphingomyelinase	GP		phosphorylate					paxillin	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
71472	19	336186	7	NULL	NULL	0	NULL	C2-ceramide	Chemical		activate					Ras	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
71473	20	336186	7	NULL	NULL	0	NULL	C2-ceramide	Chemical		activate					PI 3-K	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
71474	21	336186	7	NULL	NULL	0	NULL	C2-ceramide	Chemical		activate					SK	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
71475	22	336186	7	NULL	NULL	0	NULL	C2-ceramide	Chemical		activate					Cdc42	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
71476	23	336186	7	NULL	NULL	0	NULL	C2-ceramide	Chemical		activate					Rac	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
71477	24	336186	7	NULL	NULL	0	NULL	C2-ceramide	Chemical		activate					Rho	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
71478	25	336186	7	NULL	NULL	0	NULL	C2-ceramide	Chemical		activate					PAK	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
71479	26	336186	7	NULL	NULL	0	NULL	C2-ceramide	Chemical		phosphorylate					FAK	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
71480	27	336186	7	NULL	NULL	0	NULL	C2-ceramide	Chemical		phosphorylate					paxillin	GP		tyrosine		NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
71481	28	336186	7	NULL	NULL	0	NULL	C2-ceramide	Chemical		is a type of					cell-permeable ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
71482	29	336186	7	NULL	NULL	0	NULL	SK	GP		is					 sphingosine kinase	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
71483	30	336186	7	NULL	NULL	0	NULL	PAK	GP		is					p21-activated protein kinase	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_12_11_3618_s_32	11694593	The present work shows that TNF-alpha, sphingomyelinase, and C2-ceramide (a cell-permeable ceramide) activate Ras, PI 3-K, sphingosine kinase (SK), Cdc42, Rac, Rho, and p21-activated protein kinase (PAK) and cause the tyrosine phosphorylation of FAK and paxillin.	transcription
69426	1	336187	5	NULL	NULL	0	NULL	p38-RK	GP	activation of	is associated with		closely			ceramide	Chemical	action of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_245	9415703	In the current study, the close association of p38-RK activation with the actions of both ceramide and sphingosine raised the possibility that this signaling element could represent a common or convergent element in the ultimate apoptotic processes initiated by the two lipids; this was of particular interest inasmuch as dominant-negative suppression of c-Jun by TAM-67 was not sufficient to rule out an essential involvement of p38-RK.	transcription
69427	2	336187	5	NULL	NULL	0	NULL	p38-RK	GP	activation of	is associated with		closely			sphingosine	Chemical	action of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_245	9415703	In the current study, the close association of p38-RK activation with the actions of both ceramide and sphingosine raised the possibility that this signaling element could represent a common or convergent element in the ultimate apoptotic processes initiated by the two lipids; this was of particular interest inasmuch as dominant-negative suppression of c-Jun by TAM-67 was not sufficient to rule out an essential involvement of p38-RK.	transcription
69428	3	336187	5	NULL	NULL	0	NULL	apoptosis	Process		initiated by					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_245	9415703	In the current study, the close association of p38-RK activation with the actions of both ceramide and sphingosine raised the possibility that this signaling element could represent a common or convergent element in the ultimate apoptotic processes initiated by the two lipids; this was of particular interest inasmuch as dominant-negative suppression of c-Jun by TAM-67 was not sufficient to rule out an essential involvement of p38-RK.	transcription
69429	4	336187	5	NULL	NULL	0	NULL	apoptosis	Process		initiated by					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_245	9415703	In the current study, the close association of p38-RK activation with the actions of both ceramide and sphingosine raised the possibility that this signaling element could represent a common or convergent element in the ultimate apoptotic processes initiated by the two lipids; this was of particular interest inasmuch as dominant-negative suppression of c-Jun by TAM-67 was not sufficient to rule out an essential involvement of p38-RK.	transcription
69430	5	336187	5	NULL	NULL	NULL	NULL	p38-RK	GP		represent		possibly			statement 3	Process	common element of			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_245	9415703	In the current study, the close association of p38-RK activation with the actions of both ceramide and sphingosine raised the possibility that this signaling element could represent a common or convergent element in the ultimate apoptotic processes initiated by the two lipids; this was of particular interest inasmuch as dominant-negative suppression of c-Jun by TAM-67 was not sufficient to rule out an essential involvement of p38-RK.	transcription
69431	6	336187	5	NULL	NULL	NULL	NULL	p38-RK	GP		represent		possibly			statement 4	Process	common element of			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_245	9415703	In the current study, the close association of p38-RK activation with the actions of both ceramide and sphingosine raised the possibility that this signaling element could represent a common or convergent element in the ultimate apoptotic processes initiated by the two lipids; this was of particular interest inasmuch as dominant-negative suppression of c-Jun by TAM-67 was not sufficient to rule out an essential involvement of p38-RK.	transcription
69432	7	336187	5	NULL	NULL	NULL	NULL	p38-RK	GP		represent		possibly			statement 3	Process	convergent element of			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_245	9415703	In the current study, the close association of p38-RK activation with the actions of both ceramide and sphingosine raised the possibility that this signaling element could represent a common or convergent element in the ultimate apoptotic processes initiated by the two lipids; this was of particular interest inasmuch as dominant-negative suppression of c-Jun by TAM-67 was not sufficient to rule out an essential involvement of p38-RK.	transcription
69433	8	336187	5	NULL	NULL	NULL	NULL	p38-RK	GP		represent		possibly			statement 4	Process	convergent element of			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_245	9415703	In the current study, the close association of p38-RK activation with the actions of both ceramide and sphingosine raised the possibility that this signaling element could represent a common or convergent element in the ultimate apoptotic processes initiated by the two lipids; this was of particular interest inasmuch as dominant-negative suppression of c-Jun by TAM-67 was not sufficient to rule out an essential involvement of p38-RK.	transcription
69434	9	336187	5	NULL	NULL	0	NULL	statement 5	Process		is an alternative to					statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_245	9415703	In the current study, the close association of p38-RK activation with the actions of both ceramide and sphingosine raised the possibility that this signaling element could represent a common or convergent element in the ultimate apoptotic processes initiated by the two lipids; this was of particular interest inasmuch as dominant-negative suppression of c-Jun by TAM-67 was not sufficient to rule out an essential involvement of p38-RK.	transcription
69435	10	336187	5	NULL	NULL	0	NULL	statement 6	Process		is an alternative to					statement 8	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_245	9415703	In the current study, the close association of p38-RK activation with the actions of both ceramide and sphingosine raised the possibility that this signaling element could represent a common or convergent element in the ultimate apoptotic processes initiated by the two lipids; this was of particular interest inasmuch as dominant-negative suppression of c-Jun by TAM-67 was not sufficient to rule out an essential involvement of p38-RK.	transcription
69436	11	336187	5	NULL	NULL	0	NULL	TAM-67	GP		suppress		dominant-negative			c-Jun	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_245	9415703	In the current study, the close association of p38-RK activation with the actions of both ceramide and sphingosine raised the possibility that this signaling element could represent a common or convergent element in the ultimate apoptotic processes initiated by the two lipids; this was of particular interest inasmuch as dominant-negative suppression of c-Jun by TAM-67 was not sufficient to rule out an essential involvement of p38-RK.	transcription
71484	1	336187	7	NULL	NULL	0	NULL	p38	GP		associate with					RK	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_245	9415703	In the current study, the close association of p38-RK activation with the actions of both ceramide and sphingosine raised the possibility that this signaling element could represent a common or convergent element in the ultimate apoptotic processes initiated by the two lipids; this was of particular interest inasmuch as dominant-negative suppression of c-Jun by TAM-67 was not sufficient to rule out an essential involvement of p38-RK.	transcription
71485	2	336187	7	NULL	NULL	0	NULL	p38-RK	GP	activation of	associated with					ceramide	Chemical	actions of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_245	9415703	In the current study, the close association of p38-RK activation with the actions of both ceramide and sphingosine raised the possibility that this signaling element could represent a common or convergent element in the ultimate apoptotic processes initiated by the two lipids; this was of particular interest inasmuch as dominant-negative suppression of c-Jun by TAM-67 was not sufficient to rule out an essential involvement of p38-RK.	transcription
71486	3	336187	7	NULL	NULL	0	NULL	p38-RK	GP	activation of	associate with					sphingosine	Chemical	actions of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_245	9415703	In the current study, the close association of p38-RK activation with the actions of both ceramide and sphingosine raised the possibility that this signaling element could represent a common or convergent element in the ultimate apoptotic processes initiated by the two lipids; this was of particular interest inasmuch as dominant-negative suppression of c-Jun by TAM-67 was not sufficient to rule out an essential involvement of p38-RK.	transcription
71487	4	336187	7	NULL	NULL	0	NULL	p38-RK	GP		participate in		could			apoptotic process	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_245	9415703	In the current study, the close association of p38-RK activation with the actions of both ceramide and sphingosine raised the possibility that this signaling element could represent a common or convergent element in the ultimate apoptotic processes initiated by the two lipids; this was of particular interest inasmuch as dominant-negative suppression of c-Jun by TAM-67 was not sufficient to rule out an essential involvement of p38-RK.	transcription
71488	5	336187	7	NULL	NULL	0	NULL	ceramide	Chemical		initiates					apoptotic process	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_245	9415703	In the current study, the close association of p38-RK activation with the actions of both ceramide and sphingosine raised the possibility that this signaling element could represent a common or convergent element in the ultimate apoptotic processes initiated by the two lipids; this was of particular interest inasmuch as dominant-negative suppression of c-Jun by TAM-67 was not sufficient to rule out an essential involvement of p38-RK.	transcription
71489	6	336187	7	NULL	NULL	0	NULL	sphingosine	Chemical		initiates					apoptotic process	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_52_6_935_s_245	9415703	In the current study, the close association of p38-RK activation with the actions of both ceramide and sphingosine raised the possibility that this signaling element could represent a common or convergent element in the ultimate apoptotic processes initiated by the two lipids; this was of particular interest inasmuch as dominant-negative suppression of c-Jun by TAM-67 was not sufficient to rule out an essential involvement of p38-RK.	transcription
69464	1	336188	5	NULL	NULL	0	NULL	sphingosine kinase	GP	overexpression of	increases					SPP	Chemical	level of			NULL	C6 Cells	0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_115	11815603	Overexpression of Sphingosine Kinase in C6 Cells Increases SPP Levels-- Previously, we found that, although TNF-alpha-induced expression of iNOS and subsequent NO production were mediated in part by increases in ceramide levels, GTPCH expression and activity and levels of the iNOS cofactor BH4 were not increased in parallel ( 12).	transcription
69465	2	336188	5	NULL	NULL	0	NULL	iNOS	GP	expression of	is induced by					TNF-alpha	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_115	11815603	Overexpression of Sphingosine Kinase in C6 Cells Increases SPP Levels-- Previously, we found that, although TNF-alpha-induced expression of iNOS and subsequent NO production were mediated in part by increases in ceramide levels, GTPCH expression and activity and levels of the iNOS cofactor BH4 were not increased in parallel ( 12).	transcription
69466	3	336188	5	NULL	NULL	0	NULL	statement 2	Process		leads to		subsequently			NO	Chemical	production of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_115	11815603	Overexpression of Sphingosine Kinase in C6 Cells Increases SPP Levels-- Previously, we found that, although TNF-alpha-induced expression of iNOS and subsequent NO production were mediated in part by increases in ceramide levels, GTPCH expression and activity and levels of the iNOS cofactor BH4 were not increased in parallel ( 12).	transcription
69467	4	336188	5	NULL	NULL	0	NULL	ceramide	Chemical	increase in;;levels of	mediates					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_115	11815603	Overexpression of Sphingosine Kinase in C6 Cells Increases SPP Levels-- Previously, we found that, although TNF-alpha-induced expression of iNOS and subsequent NO production were mediated in part by increases in ceramide levels, GTPCH expression and activity and levels of the iNOS cofactor BH4 were not increased in parallel ( 12).	transcription
69468	5	336188	5	NULL	NULL	0	NULL	BH4	Chemical		is a cofactor of					iNOS	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_115	11815603	Overexpression of Sphingosine Kinase in C6 Cells Increases SPP Levels-- Previously, we found that, although TNF-alpha-induced expression of iNOS and subsequent NO production were mediated in part by increases in ceramide levels, GTPCH expression and activity and levels of the iNOS cofactor BH4 were not increased in parallel ( 12).	transcription
69469	6	336188	5	NULL	NULL	0	NULL	statement 4	Process		does not increase		parallely			GTPCH	GP	expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_115	11815603	Overexpression of Sphingosine Kinase in C6 Cells Increases SPP Levels-- Previously, we found that, although TNF-alpha-induced expression of iNOS and subsequent NO production were mediated in part by increases in ceramide levels, GTPCH expression and activity and levels of the iNOS cofactor BH4 were not increased in parallel ( 12).	transcription
69470	7	336188	5	NULL	NULL	0	NULL	statement 4	Process		does not activate		parallely			GTPCH	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_115	11815603	Overexpression of Sphingosine Kinase in C6 Cells Increases SPP Levels-- Previously, we found that, although TNF-alpha-induced expression of iNOS and subsequent NO production were mediated in part by increases in ceramide levels, GTPCH expression and activity and levels of the iNOS cofactor BH4 were not increased in parallel ( 12).	transcription
69471	8	336188	5	NULL	NULL	0	NULL	statement 4	Process		does not increase		parallely			BH4	Chemical	level of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_115	11815603	Overexpression of Sphingosine Kinase in C6 Cells Increases SPP Levels-- Previously, we found that, although TNF-alpha-induced expression of iNOS and subsequent NO production were mediated in part by increases in ceramide levels, GTPCH expression and activity and levels of the iNOS cofactor BH4 were not increased in parallel ( 12).	transcription
71490	1	336188	7	NULL	NULL	0	NULL	Sphingosine Kinase	GP	overexpression of	increase					SPP 	Chemical	levels of			NULL	C6 cells	0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_115	11815603	Overexpression of Sphingosine Kinase in C6 Cells Increases SPP Levels-- Previously, we found that, although TNF-alpha-induced expression of iNOS and subsequent NO production were mediated in part by increases in ceramide levels, GTPCH expression and activity and levels of the iNOS cofactor BH4 were not increased in parallel ( 12).	transcription
71491	2	336188	7	NULL	NULL	NULL	NULL	TNF-alpha	GP		induce					iNOS	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_115	11815603	Overexpression of Sphingosine Kinase in C6 Cells Increases SPP Levels-- Previously, we found that, although TNF-alpha-induced expression of iNOS and subsequent NO production were mediated in part by increases in ceramide levels, GTPCH expression and activity and levels of the iNOS cofactor BH4 were not increased in parallel ( 12).	transcription
71492	3	336188	7	NULL	NULL	0	NULL	statement 2	Process		produce					NO	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_115	11815603	Overexpression of Sphingosine Kinase in C6 Cells Increases SPP Levels-- Previously, we found that, although TNF-alpha-induced expression of iNOS and subsequent NO production were mediated in part by increases in ceramide levels, GTPCH expression and activity and levels of the iNOS cofactor BH4 were not increased in parallel ( 12).	transcription
71493	4	336188	7	NULL	NULL	0	NULL	statement 3	Process		mediated by		partly			ceramide	Chemical	increase in			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_115	11815603	Overexpression of Sphingosine Kinase in C6 Cells Increases SPP Levels-- Previously, we found that, although TNF-alpha-induced expression of iNOS and subsequent NO production were mediated in part by increases in ceramide levels, GTPCH expression and activity and levels of the iNOS cofactor BH4 were not increased in parallel ( 12).	transcription
71494	5	336188	7	NULL	NULL	NULL	NULL	statement 3	Process		mediated by		partly			GTPCH	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_115	11815603	Overexpression of Sphingosine Kinase in C6 Cells Increases SPP Levels-- Previously, we found that, although TNF-alpha-induced expression of iNOS and subsequent NO production were mediated in part by increases in ceramide levels, GTPCH expression and activity and levels of the iNOS cofactor BH4 were not increased in parallel ( 12).	transcription
71495	6	336188	7	NULL	NULL	0	NULL	statement 3	Process		mediated by		partly			GTPCH	GP	activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_115	11815603	Overexpression of Sphingosine Kinase in C6 Cells Increases SPP Levels-- Previously, we found that, although TNF-alpha-induced expression of iNOS and subsequent NO production were mediated in part by increases in ceramide levels, GTPCH expression and activity and levels of the iNOS cofactor BH4 were not increased in parallel ( 12).	transcription
71496	7	336188	7	NULL	NULL	0	NULL	statement 3	Process		does not increase					BH4	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_115	11815603	Overexpression of Sphingosine Kinase in C6 Cells Increases SPP Levels-- Previously, we found that, although TNF-alpha-induced expression of iNOS and subsequent NO production were mediated in part by increases in ceramide levels, GTPCH expression and activity and levels of the iNOS cofactor BH4 were not increased in parallel ( 12).	transcription
71497	8	336188	7	NULL	NULL	0	NULL	BH4 	Chemical		is a type of					 iNOS cofactor	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_15_12649_s_115	11815603	Overexpression of Sphingosine Kinase in C6 Cells Increases SPP Levels-- Previously, we found that, although TNF-alpha-induced expression of iNOS and subsequent NO production were mediated in part by increases in ceramide levels, GTPCH expression and activity and levels of the iNOS cofactor BH4 were not increased in parallel ( 12).	transcription
69472	1	336189	5	NULL	NULL	0	NULL	ceramide	Chemical		is converted to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_8_4836_s_69	9030540	First, to determine whether blocking the conversion of ceramide to sphingosine would abrogate the negative inotropic effects of TNF-alpha, freshly isolated feline cardiac myocytes were allowed to stabilize for 1 h and were then treated for 30 min at 37  degrees C with 200 units.	transcription
69473	2	336189	5	NULL	NULL	0	NULL	statement 1	Process	blocking of	abrogates		possibly			TNF-alpha	GP	negative inotropic effects of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_8_4836_s_69	9030540	First, to determine whether blocking the conversion of ceramide to sphingosine would abrogate the negative inotropic effects of TNF-alpha, freshly isolated feline cardiac myocytes were allowed to stabilize for 1 h and were then treated for 30 min at 37  degrees C with 200 units.	transcription
71498	1	336189	7	NULL	NULL	0	NULL	ceramide	Chemical		converted to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_8_4836_s_69	9030540	First, to determine whether blocking the conversion of ceramide to sphingosine would abrogate the negative inotropic effects of TNF-alpha, freshly isolated feline cardiac myocytes were allowed to stabilize for 1 h and were then treated for 30 min at 37  degrees C with 200 units.	transcription
69474	1	336190	5	NULL	NULL	0	NULL	Jurkat cells	Cell		treated with					anti-Fas antibody	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_18	10747891	Herein, we report that treatment of Jurkat cells with anti-Fas antibody induces rapid generation of ceramide immediately followed by transient production of sphingosine, both preceding cyt  c release and activation of executioner caspase-3, -6, and -7 as well as caspase-8 and Bid activation.	transcription
69475	2	336190	5	NULL	NULL	0	NULL	statement 1	Process		induce					ceramide	Chemical	rapid generation of 			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_18	10747891	Herein, we report that treatment of Jurkat cells with anti-Fas antibody induces rapid generation of ceramide immediately followed by transient production of sphingosine, both preceding cyt  c release and activation of executioner caspase-3, -6, and -7 as well as caspase-8 and Bid activation.	transcription
69476	3	336190	5	NULL	NULL	0	NULL	statement 2	Process		followed by		immediately			sphingosine	Chemical	transient production of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_18	10747891	Herein, we report that treatment of Jurkat cells with anti-Fas antibody induces rapid generation of ceramide immediately followed by transient production of sphingosine, both preceding cyt  c release and activation of executioner caspase-3, -6, and -7 as well as caspase-8 and Bid activation.	transcription
69477	4	336190	5	NULL	NULL	0	NULL	statement 2	Process		precede					cyt c	GP	release of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_18	10747891	Herein, we report that treatment of Jurkat cells with anti-Fas antibody induces rapid generation of ceramide immediately followed by transient production of sphingosine, both preceding cyt  c release and activation of executioner caspase-3, -6, and -7 as well as caspase-8 and Bid activation.	transcription
69478	5	336190	5	NULL	NULL	0	NULL	statement 3	Process		preced					cyt c	GP	release of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_18	10747891	Herein, we report that treatment of Jurkat cells with anti-Fas antibody induces rapid generation of ceramide immediately followed by transient production of sphingosine, both preceding cyt  c release and activation of executioner caspase-3, -6, and -7 as well as caspase-8 and Bid activation.	transcription
69479	6	336190	5	NULL	NULL	0	NULL	statement 2	Process		precede					caspase-3	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_18	10747891	Herein, we report that treatment of Jurkat cells with anti-Fas antibody induces rapid generation of ceramide immediately followed by transient production of sphingosine, both preceding cyt  c release and activation of executioner caspase-3, -6, and -7 as well as caspase-8 and Bid activation.	transcription
69480	7	336190	5	NULL	NULL	0	NULL	statement 3	Process		precede					caspase-3	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_18	10747891	Herein, we report that treatment of Jurkat cells with anti-Fas antibody induces rapid generation of ceramide immediately followed by transient production of sphingosine, both preceding cyt  c release and activation of executioner caspase-3, -6, and -7 as well as caspase-8 and Bid activation.	transcription
69481	8	336190	5	NULL	NULL	0	NULL	statement 2	Process		precede					caspase-6	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_18	10747891	Herein, we report that treatment of Jurkat cells with anti-Fas antibody induces rapid generation of ceramide immediately followed by transient production of sphingosine, both preceding cyt  c release and activation of executioner caspase-3, -6, and -7 as well as caspase-8 and Bid activation.	transcription
69482	9	336190	5	NULL	NULL	0	NULL	statement 3	Process		precede					caspase-6	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_18	10747891	Herein, we report that treatment of Jurkat cells with anti-Fas antibody induces rapid generation of ceramide immediately followed by transient production of sphingosine, both preceding cyt  c release and activation of executioner caspase-3, -6, and -7 as well as caspase-8 and Bid activation.	transcription
69483	10	336190	5	NULL	NULL	0	NULL	statement 2	Process		precede					caspase-7	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_18	10747891	Herein, we report that treatment of Jurkat cells with anti-Fas antibody induces rapid generation of ceramide immediately followed by transient production of sphingosine, both preceding cyt  c release and activation of executioner caspase-3, -6, and -7 as well as caspase-8 and Bid activation.	transcription
69484	11	336190	5	NULL	NULL	0	NULL	statement 3	Process		precede					caspase-7	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_18	10747891	Herein, we report that treatment of Jurkat cells with anti-Fas antibody induces rapid generation of ceramide immediately followed by transient production of sphingosine, both preceding cyt  c release and activation of executioner caspase-3, -6, and -7 as well as caspase-8 and Bid activation.	transcription
69485	12	336190	5	NULL	NULL	0	NULL	caspase-3	GP		is a type of					executioner caspase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_18	10747891	Herein, we report that treatment of Jurkat cells with anti-Fas antibody induces rapid generation of ceramide immediately followed by transient production of sphingosine, both preceding cyt  c release and activation of executioner caspase-3, -6, and -7 as well as caspase-8 and Bid activation.	transcription
69486	13	336190	5	NULL	NULL	0	NULL	caspase-6	GP		is a type of					executioner caspase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_18	10747891	Herein, we report that treatment of Jurkat cells with anti-Fas antibody induces rapid generation of ceramide immediately followed by transient production of sphingosine, both preceding cyt  c release and activation of executioner caspase-3, -6, and -7 as well as caspase-8 and Bid activation.	transcription
69487	14	336190	5	NULL	NULL	0	NULL	caspase-7	GP		is a type of					executioner caspase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_18	10747891	Herein, we report that treatment of Jurkat cells with anti-Fas antibody induces rapid generation of ceramide immediately followed by transient production of sphingosine, both preceding cyt  c release and activation of executioner caspase-3, -6, and -7 as well as caspase-8 and Bid activation.	transcription
69488	15	336190	5	NULL	NULL	0	NULL	statement 2	Process		precede					caspase-8	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_18	10747891	Herein, we report that treatment of Jurkat cells with anti-Fas antibody induces rapid generation of ceramide immediately followed by transient production of sphingosine, both preceding cyt  c release and activation of executioner caspase-3, -6, and -7 as well as caspase-8 and Bid activation.	transcription
69489	16	336190	5	NULL	NULL	0	NULL	statement 3	Process		precede					caspase-8	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_18	10747891	Herein, we report that treatment of Jurkat cells with anti-Fas antibody induces rapid generation of ceramide immediately followed by transient production of sphingosine, both preceding cyt  c release and activation of executioner caspase-3, -6, and -7 as well as caspase-8 and Bid activation.	transcription
69490	17	336190	5	NULL	NULL	0	NULL	statement 2	Process		precede					Bid	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_18	10747891	Herein, we report that treatment of Jurkat cells with anti-Fas antibody induces rapid generation of ceramide immediately followed by transient production of sphingosine, both preceding cyt  c release and activation of executioner caspase-3, -6, and -7 as well as caspase-8 and Bid activation.	transcription
69491	18	336190	5	NULL	NULL	0	NULL	statement 3	Process		precede					Bid	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_18	10747891	Herein, we report that treatment of Jurkat cells with anti-Fas antibody induces rapid generation of ceramide immediately followed by transient production of sphingosine, both preceding cyt  c release and activation of executioner caspase-3, -6, and -7 as well as caspase-8 and Bid activation.	transcription
71499	1	336190	7	NULL	NULL	0	NULL	 Jurkat cells	Cell		treated with					anti-Fas antibody	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_18	10747891	Herein, we report that treatment of Jurkat cells with anti-Fas antibody induces rapid generation of ceramide immediately followed by transient production of sphingosine, both preceding cyt  c release and activation of executioner caspase-3, -6, and -7 as well as caspase-8 and Bid activation.	transcription
71500	2	336190	7	NULL	NULL	0	NULL	statement 1	Process		induces					ceramide	Chemical	rapid generation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_18	10747891	Herein, we report that treatment of Jurkat cells with anti-Fas antibody induces rapid generation of ceramide immediately followed by transient production of sphingosine, both preceding cyt  c release and activation of executioner caspase-3, -6, and -7 as well as caspase-8 and Bid activation.	transcription
71501	3	336190	7	NULL	NULL	0	NULL	statement 2	Process		followed by		immediately			sphingosine	Chemical	transient production of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_18	10747891	Herein, we report that treatment of Jurkat cells with anti-Fas antibody induces rapid generation of ceramide immediately followed by transient production of sphingosine, both preceding cyt  c release and activation of executioner caspase-3, -6, and -7 as well as caspase-8 and Bid activation.	transcription
71502	4	336190	7	NULL	NULL	0	NULL	statement 3	Process		precede					cyt c	Chemical	release of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_18	10747891	Herein, we report that treatment of Jurkat cells with anti-Fas antibody induces rapid generation of ceramide immediately followed by transient production of sphingosine, both preceding cyt  c release and activation of executioner caspase-3, -6, and -7 as well as caspase-8 and Bid activation.	transcription
71503	5	336190	7	NULL	NULL	0	NULL	statement 3	Process		precede					caspase-3	GP	activation of executioner			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_18	10747891	Herein, we report that treatment of Jurkat cells with anti-Fas antibody induces rapid generation of ceramide immediately followed by transient production of sphingosine, both preceding cyt  c release and activation of executioner caspase-3, -6, and -7 as well as caspase-8 and Bid activation.	transcription
71504	6	336190	7	NULL	NULL	0	NULL	statement 3	Process		precede					caspase-6	GP	activation of executioner			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_18	10747891	Herein, we report that treatment of Jurkat cells with anti-Fas antibody induces rapid generation of ceramide immediately followed by transient production of sphingosine, both preceding cyt  c release and activation of executioner caspase-3, -6, and -7 as well as caspase-8 and Bid activation.	transcription
71505	7	336190	7	NULL	NULL	0	NULL	statement 3	Process		precede					caspase-7	GP	activation of executioner			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_18	10747891	Herein, we report that treatment of Jurkat cells with anti-Fas antibody induces rapid generation of ceramide immediately followed by transient production of sphingosine, both preceding cyt  c release and activation of executioner caspase-3, -6, and -7 as well as caspase-8 and Bid activation.	transcription
71506	8	336190	7	NULL	NULL	0	NULL	statement 3	Process		precede					caspase-8	GP	activation of executioner			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_18	10747891	Herein, we report that treatment of Jurkat cells with anti-Fas antibody induces rapid generation of ceramide immediately followed by transient production of sphingosine, both preceding cyt  c release and activation of executioner caspase-3, -6, and -7 as well as caspase-8 and Bid activation.	transcription
71507	9	336190	7	NULL	NULL	0	NULL	statement 3	Process		precede					Bid	GP	activation of executioner			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_18	10747891	Herein, we report that treatment of Jurkat cells with anti-Fas antibody induces rapid generation of ceramide immediately followed by transient production of sphingosine, both preceding cyt  c release and activation of executioner caspase-3, -6, and -7 as well as caspase-8 and Bid activation.	transcription
69493	1	336191	5	NULL	NULL	0	NULL	Fas	GP	cross-linking of 	triggers		rapidly			ceramide	Chemical	generation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_282	10747891	Thus, cross-linking of Fas could rapidly trigger generation of ceramide, in a caspase-dependent manner, which is then converted to sphingosine, and both sphingolipid metabolites may be involved in the translocation of cyt  c from mitochondria to the cytosol (under the control of Bcl-xL), where it can stimulate proteolytic activation of executioner caspases through caspase-9.	transcription
69494	2	336191	5	NULL	NULL	0	NULL	statement 1	Process		is dependent on					caspase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_282	10747891	Thus, cross-linking of Fas could rapidly trigger generation of ceramide, in a caspase-dependent manner, which is then converted to sphingosine, and both sphingolipid metabolites may be involved in the translocation of cyt  c from mitochondria to the cytosol (under the control of Bcl-xL), where it can stimulate proteolytic activation of executioner caspases through caspase-9.	transcription
69495	3	336191	5	NULL	NULL	0	NULL	ceramide	Chemical		is converted to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_282	10747891	Thus, cross-linking of Fas could rapidly trigger generation of ceramide, in a caspase-dependent manner, which is then converted to sphingosine, and both sphingolipid metabolites may be involved in the translocation of cyt  c from mitochondria to the cytosol (under the control of Bcl-xL), where it can stimulate proteolytic activation of executioner caspases through caspase-9.	transcription
69496	4	336191	5	NULL	NULL	0	NULL	statement 1	Process		followed by					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_282	10747891	Thus, cross-linking of Fas could rapidly trigger generation of ceramide, in a caspase-dependent manner, which is then converted to sphingosine, and both sphingolipid metabolites may be involved in the translocation of cyt  c from mitochondria to the cytosol (under the control of Bcl-xL), where it can stimulate proteolytic activation of executioner caspases through caspase-9.	transcription
69497	5	336191	5	NULL	NULL	0	NULL	cyt c	GP		is translocated from					mitochondria	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_282	10747891	Thus, cross-linking of Fas could rapidly trigger generation of ceramide, in a caspase-dependent manner, which is then converted to sphingosine, and both sphingolipid metabolites may be involved in the translocation of cyt  c from mitochondria to the cytosol (under the control of Bcl-xL), where it can stimulate proteolytic activation of executioner caspases through caspase-9.	transcription
69498	6	336191	5	NULL	NULL	0	NULL	cyt c	GP		is translocated to					cytosol	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_282	10747891	Thus, cross-linking of Fas could rapidly trigger generation of ceramide, in a caspase-dependent manner, which is then converted to sphingosine, and both sphingolipid metabolites may be involved in the translocation of cyt  c from mitochondria to the cytosol (under the control of Bcl-xL), where it can stimulate proteolytic activation of executioner caspases through caspase-9.	transcription
69499	7	336191	5	NULL	NULL	0	NULL	statement 5	Process		occurs simultaneously with					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_282	10747891	Thus, cross-linking of Fas could rapidly trigger generation of ceramide, in a caspase-dependent manner, which is then converted to sphingosine, and both sphingolipid metabolites may be involved in the translocation of cyt  c from mitochondria to the cytosol (under the control of Bcl-xL), where it can stimulate proteolytic activation of executioner caspases through caspase-9.	transcription
69500	8	336191	5	NULL	NULL	0	NULL	statement 7	Process		is controlled by					Bcl-xL	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_282	10747891	Thus, cross-linking of Fas could rapidly trigger generation of ceramide, in a caspase-dependent manner, which is then converted to sphingosine, and both sphingolipid metabolites may be involved in the translocation of cyt  c from mitochondria to the cytosol (under the control of Bcl-xL), where it can stimulate proteolytic activation of executioner caspases through caspase-9.	transcription
69501	9	336191	5	NULL	NULL	0	NULL	sphingosine	Chemical		is involved in		may be			statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_282	10747891	Thus, cross-linking of Fas could rapidly trigger generation of ceramide, in a caspase-dependent manner, which is then converted to sphingosine, and both sphingolipid metabolites may be involved in the translocation of cyt  c from mitochondria to the cytosol (under the control of Bcl-xL), where it can stimulate proteolytic activation of executioner caspases through caspase-9.	transcription
69502	10	336191	5	NULL	NULL	0	NULL	ceramide	Chemical		is involved in		may be			statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_282	10747891	Thus, cross-linking of Fas could rapidly trigger generation of ceramide, in a caspase-dependent manner, which is then converted to sphingosine, and both sphingolipid metabolites may be involved in the translocation of cyt  c from mitochondria to the cytosol (under the control of Bcl-xL), where it can stimulate proteolytic activation of executioner caspases through caspase-9.	transcription
69503	11	336191	5	NULL	NULL	0	NULL	cyt c	GP		stimulates					executioner caspases	GP	proteolytic activation of			NULL	cytosol	0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_282	10747891	Thus, cross-linking of Fas could rapidly trigger generation of ceramide, in a caspase-dependent manner, which is then converted to sphingosine, and both sphingolipid metabolites may be involved in the translocation of cyt  c from mitochondria to the cytosol (under the control of Bcl-xL), where it can stimulate proteolytic activation of executioner caspases through caspase-9.	transcription
69504	12	336191	5	NULL	NULL	0	NULL	statement 11	Process		occurs through					caspase-9	GP				NULL	cytosol	0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_282	10747891	Thus, cross-linking of Fas could rapidly trigger generation of ceramide, in a caspase-dependent manner, which is then converted to sphingosine, and both sphingolipid metabolites may be involved in the translocation of cyt  c from mitochondria to the cytosol (under the control of Bcl-xL), where it can stimulate proteolytic activation of executioner caspases through caspase-9.	transcription
71508	1	336191	7	NULL	NULL	0	NULL	Fas	GP	crosslinking of	trigger		could;;rapidly			ceramide	Chemical	generation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_282	10747891	Thus, cross-linking of Fas could rapidly trigger generation of ceramide, in a caspase-dependent manner, which is then converted to sphingosine, and both sphingolipid metabolites may be involved in the translocation of cyt  c from mitochondria to the cytosol (under the control of Bcl-xL), where it can stimulate proteolytic activation of executioner caspases through caspase-9.	transcription
71509	2	336191	7	NULL	NULL	0	NULL	statement 1	Process		depends on					caspase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_282	10747891	Thus, cross-linking of Fas could rapidly trigger generation of ceramide, in a caspase-dependent manner, which is then converted to sphingosine, and both sphingolipid metabolites may be involved in the translocation of cyt  c from mitochondria to the cytosol (under the control of Bcl-xL), where it can stimulate proteolytic activation of executioner caspases through caspase-9.	transcription
71510	3	336191	7	NULL	NULL	0	NULL	ceramide	Chemical		converted to					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_282	10747891	Thus, cross-linking of Fas could rapidly trigger generation of ceramide, in a caspase-dependent manner, which is then converted to sphingosine, and both sphingolipid metabolites may be involved in the translocation of cyt  c from mitochondria to the cytosol (under the control of Bcl-xL), where it can stimulate proteolytic activation of executioner caspases through caspase-9.	transcription
71511	4	336191	7	NULL	NULL	0	NULL	cyt c	GP		translocated from					mitochondria	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_282	10747891	Thus, cross-linking of Fas could rapidly trigger generation of ceramide, in a caspase-dependent manner, which is then converted to sphingosine, and both sphingolipid metabolites may be involved in the translocation of cyt  c from mitochondria to the cytosol (under the control of Bcl-xL), where it can stimulate proteolytic activation of executioner caspases through caspase-9.	transcription
71512	5	336191	7	NULL	NULL	NULL	NULL	cyt c	GP		translocated to					cytosol	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_282	10747891	Thus, cross-linking of Fas could rapidly trigger generation of ceramide, in a caspase-dependent manner, which is then converted to sphingosine, and both sphingolipid metabolites may be involved in the translocation of cyt  c from mitochondria to the cytosol (under the control of Bcl-xL), where it can stimulate proteolytic activation of executioner caspases through caspase-9.	transcription
71513	6	336191	7	NULL	NULL	0	NULL	statement 4	Process		occur along with					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_282	10747891	Thus, cross-linking of Fas could rapidly trigger generation of ceramide, in a caspase-dependent manner, which is then converted to sphingosine, and both sphingolipid metabolites may be involved in the translocation of cyt  c from mitochondria to the cytosol (under the control of Bcl-xL), where it can stimulate proteolytic activation of executioner caspases through caspase-9.	transcription
71514	7	336191	7	NULL	NULL	0	NULL	ceramide	Chemical		be involved in		may			statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_282	10747891	Thus, cross-linking of Fas could rapidly trigger generation of ceramide, in a caspase-dependent manner, which is then converted to sphingosine, and both sphingolipid metabolites may be involved in the translocation of cyt  c from mitochondria to the cytosol (under the control of Bcl-xL), where it can stimulate proteolytic activation of executioner caspases through caspase-9.	transcription
71515	8	336191	7	NULL	NULL	0	NULL	sphingosine	Chemical		be involved in		may			statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_282	10747891	Thus, cross-linking of Fas could rapidly trigger generation of ceramide, in a caspase-dependent manner, which is then converted to sphingosine, and both sphingolipid metabolites may be involved in the translocation of cyt  c from mitochondria to the cytosol (under the control of Bcl-xL), where it can stimulate proteolytic activation of executioner caspases through caspase-9.	transcription
71516	9	336191	7	NULL	NULL	0	NULL	statement 6	Process		stimulate					executioner caspases	GP	proteolytic activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_282	10747891	Thus, cross-linking of Fas could rapidly trigger generation of ceramide, in a caspase-dependent manner, which is then converted to sphingosine, and both sphingolipid metabolites may be involved in the translocation of cyt  c from mitochondria to the cytosol (under the control of Bcl-xL), where it can stimulate proteolytic activation of executioner caspases through caspase-9.	transcription
71517	10	336191	7	NULL	NULL	0	NULL	statement 9	Process		occur through					caspase-9	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_21_15691_s_282	10747891	Thus, cross-linking of Fas could rapidly trigger generation of ceramide, in a caspase-dependent manner, which is then converted to sphingosine, and both sphingolipid metabolites may be involved in the translocation of cyt  c from mitochondria to the cytosol (under the control of Bcl-xL), where it can stimulate proteolytic activation of executioner caspases through caspase-9.	transcription
69505	1	336192	5	NULL	NULL	0	NULL	apoptosis	Process		is mediated by					Fas	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_71	9446602	Sphingosine 1-Phosphate and TPA Inhibit Fas- and C 2 -Ceramide-mediated Apoptosis--  s described previously ( 7,  18,  20), Jurkat cells treated with Fas antibody underwent extensive cell death within 3 h as measured by the quantitative DNA fragmentation assay (Fig.  1 A).	transcription
69506	2	336192	5	NULL	NULL	0	NULL	apoptosis	Process		is mediated by					C 2 -Ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_71	9446602	Sphingosine 1-Phosphate and TPA Inhibit Fas- and C 2 -Ceramide-mediated Apoptosis--  s described previously ( 7,  18,  20), Jurkat cells treated with Fas antibody underwent extensive cell death within 3 h as measured by the quantitative DNA fragmentation assay (Fig.  1 A).	transcription
69507	3	336192	5	NULL	NULL	0	NULL	Sphingosine 1-Phosphate	Chemical		inhibits					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_71	9446602	Sphingosine 1-Phosphate and TPA Inhibit Fas- and C 2 -Ceramide-mediated Apoptosis--  s described previously ( 7,  18,  20), Jurkat cells treated with Fas antibody underwent extensive cell death within 3 h as measured by the quantitative DNA fragmentation assay (Fig.  1 A).	transcription
69508	4	336192	5	NULL	NULL	0	NULL	Sphingosine 1-Phosphate	Chemical		inhibits					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_71	9446602	Sphingosine 1-Phosphate and TPA Inhibit Fas- and C 2 -Ceramide-mediated Apoptosis--  s described previously ( 7,  18,  20), Jurkat cells treated with Fas antibody underwent extensive cell death within 3 h as measured by the quantitative DNA fragmentation assay (Fig.  1 A).	transcription
69509	5	336192	5	NULL	NULL	0	NULL	TPA	Chemical		inhibits					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_71	9446602	Sphingosine 1-Phosphate and TPA Inhibit Fas- and C 2 -Ceramide-mediated Apoptosis--  s described previously ( 7,  18,  20), Jurkat cells treated with Fas antibody underwent extensive cell death within 3 h as measured by the quantitative DNA fragmentation assay (Fig.  1 A).	transcription
69510	6	336192	5	NULL	NULL	0	NULL	TPA	Chemical		inhibits					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_71	9446602	Sphingosine 1-Phosphate and TPA Inhibit Fas- and C 2 -Ceramide-mediated Apoptosis--  s described previously ( 7,  18,  20), Jurkat cells treated with Fas antibody underwent extensive cell death within 3 h as measured by the quantitative DNA fragmentation assay (Fig.  1 A).	transcription
71518	1	336192	7	NULL	NULL	0	NULL	Fas	GP		mediates					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_71	9446602	Sphingosine 1-Phosphate and TPA Inhibit Fas- and C 2 -Ceramide-mediated Apoptosis--  s described previously ( 7,  18,  20), Jurkat cells treated with Fas antibody underwent extensive cell death within 3 h as measured by the quantitative DNA fragmentation assay (Fig.  1 A).	transcription
71519	2	336192	7	NULL	NULL	0	NULL	C 2 -Ceramide	Chemical		mediates					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_71	9446602	Sphingosine 1-Phosphate and TPA Inhibit Fas- and C 2 -Ceramide-mediated Apoptosis--  s described previously ( 7,  18,  20), Jurkat cells treated with Fas antibody underwent extensive cell death within 3 h as measured by the quantitative DNA fragmentation assay (Fig.  1 A).	transcription
71520	3	336192	7	NULL	NULL	0	NULL	Sphingosine 1-Phosphate	Chemical		inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_71	9446602	Sphingosine 1-Phosphate and TPA Inhibit Fas- and C 2 -Ceramide-mediated Apoptosis--  s described previously ( 7,  18,  20), Jurkat cells treated with Fas antibody underwent extensive cell death within 3 h as measured by the quantitative DNA fragmentation assay (Fig.  1 A).	transcription
71521	4	336192	7	NULL	NULL	0	NULL	Sphingosine 1-Phosphate	Chemical		inhibit					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_71	9446602	Sphingosine 1-Phosphate and TPA Inhibit Fas- and C 2 -Ceramide-mediated Apoptosis--  s described previously ( 7,  18,  20), Jurkat cells treated with Fas antibody underwent extensive cell death within 3 h as measured by the quantitative DNA fragmentation assay (Fig.  1 A).	transcription
71522	5	336192	7	NULL	NULL	0	NULL	TPA	Chemical		inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_71	9446602	Sphingosine 1-Phosphate and TPA Inhibit Fas- and C 2 -Ceramide-mediated Apoptosis--  s described previously ( 7,  18,  20), Jurkat cells treated with Fas antibody underwent extensive cell death within 3 h as measured by the quantitative DNA fragmentation assay (Fig.  1 A).	transcription
71523	6	336192	7	NULL	NULL	0	NULL	TPA	Chemical		inhibit					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_5_2910_s_71	9446602	Sphingosine 1-Phosphate and TPA Inhibit Fas- and C 2 -Ceramide-mediated Apoptosis--  s described previously ( 7,  18,  20), Jurkat cells treated with Fas antibody underwent extensive cell death within 3 h as measured by the quantitative DNA fragmentation assay (Fig.  1 A).	transcription
69511	1	336193	5	NULL	NULL	NULL	NULL	p125FAK	GP		undergoes					phosphorylation	Process		tyrosine		NULL	Swiss 3T3 cells	NULL	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_145	9096129	However, both sphingosine and ceramide stimulate actin stress fiber formation and focal adhesion assembly in Swiss 3T3 cells as a result of tyrosine phosphorylation of p125FAK and paxillin (Seufferlein and Rozengurt, 1994  ), which are early events in the action of diverse signaling pathways that lead to alterations in cytoskeletal organization.	transcription
69512	2	336193	5	NULL	NULL	NULL	NULL	paxillin	GP		undergoes					phosphorylation	Process		tyrosine		NULL	Swiss 3T3 cells	NULL	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_145	9096129	However, both sphingosine and ceramide stimulate actin stress fiber formation and focal adhesion assembly in Swiss 3T3 cells as a result of tyrosine phosphorylation of p125FAK and paxillin (Seufferlein and Rozengurt, 1994  ), which are early events in the action of diverse signaling pathways that lead to alterations in cytoskeletal organization.	transcription
69513	3	336193	5	NULL	NULL	0	NULL	sphingosine	Chemical		stimulates					actin stress fiber	CellComponent	formation of			NULL	Swiss 3T3 cells	0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_145	9096129	However, both sphingosine and ceramide stimulate actin stress fiber formation and focal adhesion assembly in Swiss 3T3 cells as a result of tyrosine phosphorylation of p125FAK and paxillin (Seufferlein and Rozengurt, 1994  ), which are early events in the action of diverse signaling pathways that lead to alterations in cytoskeletal organization.	transcription
69514	4	336193	5	NULL	NULL	0	NULL	ceramide	Chemical		stimulates					actin stress fiber	CellComponent	formation of			NULL	Swiss 3T3 cells	0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_145	9096129	However, both sphingosine and ceramide stimulate actin stress fiber formation and focal adhesion assembly in Swiss 3T3 cells as a result of tyrosine phosphorylation of p125FAK and paxillin (Seufferlein and Rozengurt, 1994  ), which are early events in the action of diverse signaling pathways that lead to alterations in cytoskeletal organization.	transcription
69515	5	336193	5	NULL	NULL	NULL	NULL	sphingosine	Chemical		stimulates					focal adhesion	CellComponent	assembly of			NULL	Swiss 3T3 cells	NULL	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_145	9096129	However, both sphingosine and ceramide stimulate actin stress fiber formation and focal adhesion assembly in Swiss 3T3 cells as a result of tyrosine phosphorylation of p125FAK and paxillin (Seufferlein and Rozengurt, 1994  ), which are early events in the action of diverse signaling pathways that lead to alterations in cytoskeletal organization.	transcription
69517	6	336193	5	NULL	NULL	0	NULL	ceramide	Chemical		stimulates					focal adhesion	CellComponent	assembly of			NULL	Swiss 3T3 cells	0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_145	9096129	However, both sphingosine and ceramide stimulate actin stress fiber formation and focal adhesion assembly in Swiss 3T3 cells as a result of tyrosine phosphorylation of p125FAK and paxillin (Seufferlein and Rozengurt, 1994  ), which are early events in the action of diverse signaling pathways that lead to alterations in cytoskeletal organization.	transcription
69518	7	336193	5	NULL	NULL	0	NULL	statement 1	Process		leads to					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_145	9096129	However, both sphingosine and ceramide stimulate actin stress fiber formation and focal adhesion assembly in Swiss 3T3 cells as a result of tyrosine phosphorylation of p125FAK and paxillin (Seufferlein and Rozengurt, 1994  ), which are early events in the action of diverse signaling pathways that lead to alterations in cytoskeletal organization.	transcription
69519	8	336193	5	NULL	NULL	NULL	NULL	statement 1	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_145	9096129	However, both sphingosine and ceramide stimulate actin stress fiber formation and focal adhesion assembly in Swiss 3T3 cells as a result of tyrosine phosphorylation of p125FAK and paxillin (Seufferlein and Rozengurt, 1994  ), which are early events in the action of diverse signaling pathways that lead to alterations in cytoskeletal organization.	transcription
69520	9	336193	5	NULL	NULL	0	NULL	statement 1	Process		leads to					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_145	9096129	However, both sphingosine and ceramide stimulate actin stress fiber formation and focal adhesion assembly in Swiss 3T3 cells as a result of tyrosine phosphorylation of p125FAK and paxillin (Seufferlein and Rozengurt, 1994  ), which are early events in the action of diverse signaling pathways that lead to alterations in cytoskeletal organization.	transcription
69521	10	336193	5	NULL	NULL	0	NULL	statement 1	Process		leads to					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_145	9096129	However, both sphingosine and ceramide stimulate actin stress fiber formation and focal adhesion assembly in Swiss 3T3 cells as a result of tyrosine phosphorylation of p125FAK and paxillin (Seufferlein and Rozengurt, 1994  ), which are early events in the action of diverse signaling pathways that lead to alterations in cytoskeletal organization.	transcription
69522	11	336193	5	NULL	NULL	0	NULL	statement 2	Process		leads to					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_145	9096129	However, both sphingosine and ceramide stimulate actin stress fiber formation and focal adhesion assembly in Swiss 3T3 cells as a result of tyrosine phosphorylation of p125FAK and paxillin (Seufferlein and Rozengurt, 1994  ), which are early events in the action of diverse signaling pathways that lead to alterations in cytoskeletal organization.	transcription
69523	12	336193	5	NULL	NULL	0	NULL	statement 2	Process		leads to					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_145	9096129	However, both sphingosine and ceramide stimulate actin stress fiber formation and focal adhesion assembly in Swiss 3T3 cells as a result of tyrosine phosphorylation of p125FAK and paxillin (Seufferlein and Rozengurt, 1994  ), which are early events in the action of diverse signaling pathways that lead to alterations in cytoskeletal organization.	transcription
69524	13	336193	5	NULL	NULL	0	NULL	statement 2	Process		leads to					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_145	9096129	However, both sphingosine and ceramide stimulate actin stress fiber formation and focal adhesion assembly in Swiss 3T3 cells as a result of tyrosine phosphorylation of p125FAK and paxillin (Seufferlein and Rozengurt, 1994  ), which are early events in the action of diverse signaling pathways that lead to alterations in cytoskeletal organization.	transcription
69525	14	336193	5	NULL	NULL	0	NULL	statement 2	Process		leads to					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_145	9096129	However, both sphingosine and ceramide stimulate actin stress fiber formation and focal adhesion assembly in Swiss 3T3 cells as a result of tyrosine phosphorylation of p125FAK and paxillin (Seufferlein and Rozengurt, 1994  ), which are early events in the action of diverse signaling pathways that lead to alterations in cytoskeletal organization.	transcription
71524	1	336193	7	NULL	NULL	NULL	NULL	sphingosine	Chemical		stimulate					actin stress fiber	GP	formation of			NULL	Swiss 3T3 cells	NULL	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_145	9096129	However, both sphingosine and ceramide stimulate actin stress fiber formation and focal adhesion assembly in Swiss 3T3 cells as a result of tyrosine phosphorylation of p125FAK and paxillin (Seufferlein and Rozengurt, 1994  ), which are early events in the action of diverse signaling pathways that lead to alterations in cytoskeletal organization.	transcription
71525	2	336193	7	NULL	NULL	0	NULL	ceramide	Chemical		stimulate					actin stress fiber	GP	formation of			NULL	Swiss 3T3 cells	0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_145	9096129	However, both sphingosine and ceramide stimulate actin stress fiber formation and focal adhesion assembly in Swiss 3T3 cells as a result of tyrosine phosphorylation of p125FAK and paxillin (Seufferlein and Rozengurt, 1994  ), which are early events in the action of diverse signaling pathways that lead to alterations in cytoskeletal organization.	transcription
71526	3	336193	7	NULL	NULL	0	NULL	sphingosine	Chemical		stimulate					focal adhesion assembly	Process				NULL	Swiss 3T3 cells	0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_145	9096129	However, both sphingosine and ceramide stimulate actin stress fiber formation and focal adhesion assembly in Swiss 3T3 cells as a result of tyrosine phosphorylation of p125FAK and paxillin (Seufferlein and Rozengurt, 1994  ), which are early events in the action of diverse signaling pathways that lead to alterations in cytoskeletal organization.	transcription
71527	4	336193	7	NULL	NULL	0	NULL	ceramide	Chemical		stimulate					focal adhesion assembly	Process				NULL	Swiss 3T3 cells	0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_145	9096129	However, both sphingosine and ceramide stimulate actin stress fiber formation and focal adhesion assembly in Swiss 3T3 cells as a result of tyrosine phosphorylation of p125FAK and paxillin (Seufferlein and Rozengurt, 1994  ), which are early events in the action of diverse signaling pathways that lead to alterations in cytoskeletal organization.	transcription
71528	5	336193	7	NULL	NULL	0	NULL	statement 1	Process		as a result of					p125FAK	GP	phosphorylation of	tyrosine 		NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_145	9096129	However, both sphingosine and ceramide stimulate actin stress fiber formation and focal adhesion assembly in Swiss 3T3 cells as a result of tyrosine phosphorylation of p125FAK and paxillin (Seufferlein and Rozengurt, 1994  ), which are early events in the action of diverse signaling pathways that lead to alterations in cytoskeletal organization.	transcription
71529	6	336193	7	NULL	NULL	NULL	NULL	statement 1	Process		as a result of					paxillin	GP	phosphorylation of	tyrosine		NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_145	9096129	However, both sphingosine and ceramide stimulate actin stress fiber formation and focal adhesion assembly in Swiss 3T3 cells as a result of tyrosine phosphorylation of p125FAK and paxillin (Seufferlein and Rozengurt, 1994  ), which are early events in the action of diverse signaling pathways that lead to alterations in cytoskeletal organization.	transcription
71530	7	336193	7	NULL	NULL	0	NULL	statement 2	Process		as a result of					p125FAK	GP	phosphorylation of	tyrosine		NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_145	9096129	However, both sphingosine and ceramide stimulate actin stress fiber formation and focal adhesion assembly in Swiss 3T3 cells as a result of tyrosine phosphorylation of p125FAK and paxillin (Seufferlein and Rozengurt, 1994  ), which are early events in the action of diverse signaling pathways that lead to alterations in cytoskeletal organization.	transcription
71531	8	336193	7	NULL	NULL	0	NULL	statement 2	Process		as a result of					paxillin	GP	phosphorylation of	tyrosine		NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_145	9096129	However, both sphingosine and ceramide stimulate actin stress fiber formation and focal adhesion assembly in Swiss 3T3 cells as a result of tyrosine phosphorylation of p125FAK and paxillin (Seufferlein and Rozengurt, 1994  ), which are early events in the action of diverse signaling pathways that lead to alterations in cytoskeletal organization.	transcription
71532	9	336193	7	NULL	NULL	0	NULL	statement 3	Process		as a result of					p125FAK	GP	phosphorylation of	tyrosine		NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_145	9096129	However, both sphingosine and ceramide stimulate actin stress fiber formation and focal adhesion assembly in Swiss 3T3 cells as a result of tyrosine phosphorylation of p125FAK and paxillin (Seufferlein and Rozengurt, 1994  ), which are early events in the action of diverse signaling pathways that lead to alterations in cytoskeletal organization.	transcription
71533	10	336193	7	NULL	NULL	0	NULL	statement 3	Process		as a result of					paxillin	GP	phosphorylation of	tyrosine		NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_145	9096129	However, both sphingosine and ceramide stimulate actin stress fiber formation and focal adhesion assembly in Swiss 3T3 cells as a result of tyrosine phosphorylation of p125FAK and paxillin (Seufferlein and Rozengurt, 1994  ), which are early events in the action of diverse signaling pathways that lead to alterations in cytoskeletal organization.	transcription
71534	11	336193	7	NULL	NULL	0	NULL	statement 4	Process		as a result of					p125FAK	GP	phosphorylation of	tyrosine		NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_145	9096129	However, both sphingosine and ceramide stimulate actin stress fiber formation and focal adhesion assembly in Swiss 3T3 cells as a result of tyrosine phosphorylation of p125FAK and paxillin (Seufferlein and Rozengurt, 1994  ), which are early events in the action of diverse signaling pathways that lead to alterations in cytoskeletal organization.	transcription
71535	12	336193	7	NULL	NULL	0	NULL	statement 4	Process		as a result of					paxillin	GP	phosphorylation of	tyrosine		NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_145	9096129	However, both sphingosine and ceramide stimulate actin stress fiber formation and focal adhesion assembly in Swiss 3T3 cells as a result of tyrosine phosphorylation of p125FAK and paxillin (Seufferlein and Rozengurt, 1994  ), which are early events in the action of diverse signaling pathways that lead to alterations in cytoskeletal organization.	transcription
71536	13	336193	7	NULL	NULL	NULL	NULL	statement 1	Process		 events in the		early			signaling pathways	Process	action of diverse			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_145	9096129	However, both sphingosine and ceramide stimulate actin stress fiber formation and focal adhesion assembly in Swiss 3T3 cells as a result of tyrosine phosphorylation of p125FAK and paxillin (Seufferlein and Rozengurt, 1994  ), which are early events in the action of diverse signaling pathways that lead to alterations in cytoskeletal organization.	transcription
71537	14	336193	7	NULL	NULL	0	NULL	statement 2	Process		events in the		early			signaling pathways	Process	action of diverse			NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_145	9096129	However, both sphingosine and ceramide stimulate actin stress fiber formation and focal adhesion assembly in Swiss 3T3 cells as a result of tyrosine phosphorylation of p125FAK and paxillin (Seufferlein and Rozengurt, 1994  ), which are early events in the action of diverse signaling pathways that lead to alterations in cytoskeletal organization.	transcription
71538	15	336193	7	NULL	NULL	0	NULL	statement 13	Process		leads to					cytoskeletal organization	Process	alterations in			NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_145	9096129	However, both sphingosine and ceramide stimulate actin stress fiber formation and focal adhesion assembly in Swiss 3T3 cells as a result of tyrosine phosphorylation of p125FAK and paxillin (Seufferlein and Rozengurt, 1994  ), which are early events in the action of diverse signaling pathways that lead to alterations in cytoskeletal organization.	transcription
71539	16	336193	7	NULL	NULL	0	NULL	statement 14	Process		leads to					cytoskeletal organization	Process	alterations in			NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_145	9096129	However, both sphingosine and ceramide stimulate actin stress fiber formation and focal adhesion assembly in Swiss 3T3 cells as a result of tyrosine phosphorylation of p125FAK and paxillin (Seufferlein and Rozengurt, 1994  ), which are early events in the action of diverse signaling pathways that lead to alterations in cytoskeletal organization.	transcription
69526	1	336194	5	NULL	NULL	0	NULL	SAPK	GP		induce					apoptosis	Process				NULL	U937 cells	0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_186	10454518	Direct comparison of SAPK and AP1 involvement in the induction of apoptosis in U937 cells by these cytotoxic messengers revealed that ceramide lethality is markedly attenuated by disruption of the SEK/JNK module or interference with AP1 (Jarvis et al., 1997  ), whereas sphingosine lethality is unaffected by such manipulations (Jarvis et al., 1997  ).	transcription
69527	2	336194	5	NULL	NULL	NULL	NULL	AP1	GP		is involved in					apoptosis	Process				NULL	U937 cells	NULL	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_186	10454518	Direct comparison of SAPK and AP1 involvement in the induction of apoptosis in U937 cells by these cytotoxic messengers revealed that ceramide lethality is markedly attenuated by disruption of the SEK/JNK module or interference with AP1 (Jarvis et al., 1997  ), whereas sphingosine lethality is unaffected by such manipulations (Jarvis et al., 1997  ).	transcription
69528	3	336194	5	NULL	NULL	0	NULL	ceramide lethality	Process		attenuated by		markedly			SEK/JNK module	Process	disruption of			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_186	10454518	Direct comparison of SAPK and AP1 involvement in the induction of apoptosis in U937 cells by these cytotoxic messengers revealed that ceramide lethality is markedly attenuated by disruption of the SEK/JNK module or interference with AP1 (Jarvis et al., 1997  ), whereas sphingosine lethality is unaffected by such manipulations (Jarvis et al., 1997  ).	transcription
69529	4	336194	5	NULL	NULL	0	NULL	ceramide lethality	Process		attenuated by		markedly			AP1	GP	interference of			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_186	10454518	Direct comparison of SAPK and AP1 involvement in the induction of apoptosis in U937 cells by these cytotoxic messengers revealed that ceramide lethality is markedly attenuated by disruption of the SEK/JNK module or interference with AP1 (Jarvis et al., 1997  ), whereas sphingosine lethality is unaffected by such manipulations (Jarvis et al., 1997  ).	transcription
71548	1	336194	7	NULL	NULL	0	NULL	SAPK	GP		is involved in					apoptosis	Process	induction of			NULL	U937 cells	0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_186	10454518	Direct comparison of SAPK and AP1 involvement in the induction of apoptosis in U937 cells by these cytotoxic messengers revealed that ceramide lethality is markedly attenuated by disruption of the SEK/JNK module or interference with AP1 (Jarvis et al., 1997  ), whereas sphingosine lethality is unaffected by such manipulations (Jarvis et al., 1997  ).	transcription
71549	2	336194	7	NULL	NULL	0	NULL	AP1	GP		is involved in					apoptosis	Process	induction of			NULL	U937 cells	0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_186	10454518	Direct comparison of SAPK and AP1 involvement in the induction of apoptosis in U937 cells by these cytotoxic messengers revealed that ceramide lethality is markedly attenuated by disruption of the SEK/JNK module or interference with AP1 (Jarvis et al., 1997  ), whereas sphingosine lethality is unaffected by such manipulations (Jarvis et al., 1997  ).	transcription
71550	3	336194	7	NULL	NULL	0	NULL	SAPK	GP		is a type of					cytotoxic messengers	GP				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_186	10454518	Direct comparison of SAPK and AP1 involvement in the induction of apoptosis in U937 cells by these cytotoxic messengers revealed that ceramide lethality is markedly attenuated by disruption of the SEK/JNK module or interference with AP1 (Jarvis et al., 1997  ), whereas sphingosine lethality is unaffected by such manipulations (Jarvis et al., 1997  ).	transcription
71551	4	336194	7	NULL	NULL	0	NULL	AP1	GP		is a type of					cytotoxic messengers	GP				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_186	10454518	Direct comparison of SAPK and AP1 involvement in the induction of apoptosis in U937 cells by these cytotoxic messengers revealed that ceramide lethality is markedly attenuated by disruption of the SEK/JNK module or interference with AP1 (Jarvis et al., 1997  ), whereas sphingosine lethality is unaffected by such manipulations (Jarvis et al., 1997  ).	transcription
71552	5	336194	7	NULL	NULL	0	NULL	 ceramide	Chemical	lethality of	attenuated by		markedly			SEK/JNK module	GP	disruption of			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_186	10454518	Direct comparison of SAPK and AP1 involvement in the induction of apoptosis in U937 cells by these cytotoxic messengers revealed that ceramide lethality is markedly attenuated by disruption of the SEK/JNK module or interference with AP1 (Jarvis et al., 1997  ), whereas sphingosine lethality is unaffected by such manipulations (Jarvis et al., 1997  ).	transcription
71553	6	336194	7	NULL	NULL	0	NULL	ceramide	Chemical	lethality of	attenuated by		markedly			AP1	GP	interference with			NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_186	10454518	Direct comparison of SAPK and AP1 involvement in the induction of apoptosis in U937 cells by these cytotoxic messengers revealed that ceramide lethality is markedly attenuated by disruption of the SEK/JNK module or interference with AP1 (Jarvis et al., 1997  ), whereas sphingosine lethality is unaffected by such manipulations (Jarvis et al., 1997  ).	transcription
71554	7	336194	7	NULL	NULL	0	NULL	sphingosine	Chemical	lethality of	does not affect					SEK/JNK module	GP				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_186	10454518	Direct comparison of SAPK and AP1 involvement in the induction of apoptosis in U937 cells by these cytotoxic messengers revealed that ceramide lethality is markedly attenuated by disruption of the SEK/JNK module or interference with AP1 (Jarvis et al., 1997  ), whereas sphingosine lethality is unaffected by such manipulations (Jarvis et al., 1997  ).	transcription
71555	8	336194	7	NULL	NULL	0	NULL	sphingosine	Chemical	lethality of	does not affect					AP1	GP				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_186	10454518	Direct comparison of SAPK and AP1 involvement in the induction of apoptosis in U937 cells by these cytotoxic messengers revealed that ceramide lethality is markedly attenuated by disruption of the SEK/JNK module or interference with AP1 (Jarvis et al., 1997  ), whereas sphingosine lethality is unaffected by such manipulations (Jarvis et al., 1997  ).	transcription
71556	9	336194	7	NULL	NULL	0	NULL	statement 1	Process		reveals					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_186	10454518	Direct comparison of SAPK and AP1 involvement in the induction of apoptosis in U937 cells by these cytotoxic messengers revealed that ceramide lethality is markedly attenuated by disruption of the SEK/JNK module or interference with AP1 (Jarvis et al., 1997  ), whereas sphingosine lethality is unaffected by such manipulations (Jarvis et al., 1997  ).	transcription
71557	10	336194	7	NULL	NULL	0	NULL	statement 1	Process		reveals					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_186	10454518	Direct comparison of SAPK and AP1 involvement in the induction of apoptosis in U937 cells by these cytotoxic messengers revealed that ceramide lethality is markedly attenuated by disruption of the SEK/JNK module or interference with AP1 (Jarvis et al., 1997  ), whereas sphingosine lethality is unaffected by such manipulations (Jarvis et al., 1997  ).	transcription
71558	11	336194	7	NULL	NULL	0	NULL	statement 2	Process		reveals					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_186	10454518	Direct comparison of SAPK and AP1 involvement in the induction of apoptosis in U937 cells by these cytotoxic messengers revealed that ceramide lethality is markedly attenuated by disruption of the SEK/JNK module or interference with AP1 (Jarvis et al., 1997  ), whereas sphingosine lethality is unaffected by such manipulations (Jarvis et al., 1997  ).	transcription
71559	12	336194	7	NULL	NULL	0	NULL	statement 2	Process		reveals					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_jpharmacolexpther_290_3_1384_s_186	10454518	Direct comparison of SAPK and AP1 involvement in the induction of apoptosis in U937 cells by these cytotoxic messengers revealed that ceramide lethality is markedly attenuated by disruption of the SEK/JNK module or interference with AP1 (Jarvis et al., 1997  ), whereas sphingosine lethality is unaffected by such manipulations (Jarvis et al., 1997  ).	transcription
69530	1	336196	5	NULL	NULL	0	NULL	arachidonic acid	Chemical		is the product of					PLA2	GP				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1735_1_68_s_17	15950537	Thus, arachidonic acid, the product  of PLA2, induces SM hydrolysis   [16], the cytosolic PLA2 can be inhibited by sphingosine   [17] and by SM   [17] and   [18], the inhibition by SM can be removed by sphingomyelinase   [18], ceramide accelerates the translocation of calcium-dependent PLA2 from cytosol to membranes in platelets   [19], and sphingosine and sphinganine directly inhibit PLA2  [20].	transcription
69531	2	336196	5	NULL	NULL	0	NULL	arachidonic acid	Chemical		hydrolyzes					SM	Chemical				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1735_1_68_s_17	15950537	Thus, arachidonic acid, the product  of PLA2, induces SM hydrolysis   [16], the cytosolic PLA2 can be inhibited by sphingosine   [17] and by SM   [17] and   [18], the inhibition by SM can be removed by sphingomyelinase   [18], ceramide accelerates the translocation of calcium-dependent PLA2 from cytosol to membranes in platelets   [19], and sphingosine and sphinganine directly inhibit PLA2  [20].	transcription
69532	3	336196	5	NULL	NULL	0	NULL	PLA2	GP	cytosolic	is inhibited by					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1735_1_68_s_17	15950537	Thus, arachidonic acid, the product  of PLA2, induces SM hydrolysis   [16], the cytosolic PLA2 can be inhibited by sphingosine   [17] and by SM   [17] and   [18], the inhibition by SM can be removed by sphingomyelinase   [18], ceramide accelerates the translocation of calcium-dependent PLA2 from cytosol to membranes in platelets   [19], and sphingosine and sphinganine directly inhibit PLA2  [20].	transcription
69533	4	336196	5	NULL	NULL	0	NULL	PLA2	GP	cytosolic	is inhibited by					SM	Chemical				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1735_1_68_s_17	15950537	Thus, arachidonic acid, the product  of PLA2, induces SM hydrolysis   [16], the cytosolic PLA2 can be inhibited by sphingosine   [17] and by SM   [17] and   [18], the inhibition by SM can be removed by sphingomyelinase   [18], ceramide accelerates the translocation of calcium-dependent PLA2 from cytosol to membranes in platelets   [19], and sphingosine and sphinganine directly inhibit PLA2  [20].	transcription
69534	5	336196	5	NULL	NULL	0	NULL	sphingomyelinase	GP		removes					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1735_1_68_s_17	15950537	Thus, arachidonic acid, the product  of PLA2, induces SM hydrolysis   [16], the cytosolic PLA2 can be inhibited by sphingosine   [17] and by SM   [17] and   [18], the inhibition by SM can be removed by sphingomyelinase   [18], ceramide accelerates the translocation of calcium-dependent PLA2 from cytosol to membranes in platelets   [19], and sphingosine and sphinganine directly inhibit PLA2  [20].	transcription
69535	6	336196	5	NULL	NULL	0	NULL	PLA2	GP	calcium-dependent	is translocated from					cytosol	CellComponent				NULL	platelets	0	NULL	NULL	NULL	gw70_biochimbiophysacta_1735_1_68_s_17	15950537	Thus, arachidonic acid, the product  of PLA2, induces SM hydrolysis   [16], the cytosolic PLA2 can be inhibited by sphingosine   [17] and by SM   [17] and   [18], the inhibition by SM can be removed by sphingomyelinase   [18], ceramide accelerates the translocation of calcium-dependent PLA2 from cytosol to membranes in platelets   [19], and sphingosine and sphinganine directly inhibit PLA2  [20].	transcription
69536	7	336196	5	NULL	NULL	0	NULL	PLA2	GP	calcium-dependent	is translocated to					membranes	CellComponent				NULL	platelets	0	NULL	NULL	NULL	gw70_biochimbiophysacta_1735_1_68_s_17	15950537	Thus, arachidonic acid, the product  of PLA2, induces SM hydrolysis   [16], the cytosolic PLA2 can be inhibited by sphingosine   [17] and by SM   [17] and   [18], the inhibition by SM can be removed by sphingomyelinase   [18], ceramide accelerates the translocation of calcium-dependent PLA2 from cytosol to membranes in platelets   [19], and sphingosine and sphinganine directly inhibit PLA2  [20].	transcription
69537	8	336196	5	NULL	NULL	0	NULL	statement 6	Process		occurs along with					statement 7	Process				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1735_1_68_s_17	15950537	Thus, arachidonic acid, the product  of PLA2, induces SM hydrolysis   [16], the cytosolic PLA2 can be inhibited by sphingosine   [17] and by SM   [17] and   [18], the inhibition by SM can be removed by sphingomyelinase   [18], ceramide accelerates the translocation of calcium-dependent PLA2 from cytosol to membranes in platelets   [19], and sphingosine and sphinganine directly inhibit PLA2  [20].	transcription
69539	9	336196	5	NULL	NULL	0	NULL	ceramide	Chemical		accelerates					statement 6	Process				NULL	platelets	0	NULL	NULL	NULL	gw70_biochimbiophysacta_1735_1_68_s_17	15950537	Thus, arachidonic acid, the product  of PLA2, induces SM hydrolysis   [16], the cytosolic PLA2 can be inhibited by sphingosine   [17] and by SM   [17] and   [18], the inhibition by SM can be removed by sphingomyelinase   [18], ceramide accelerates the translocation of calcium-dependent PLA2 from cytosol to membranes in platelets   [19], and sphingosine and sphinganine directly inhibit PLA2  [20].	transcription
69540	10	336196	5	NULL	NULL	0	NULL	ceramide	Chemical		accelerates					statement 7	Process				NULL	platelets	0	NULL	NULL	NULL	gw70_biochimbiophysacta_1735_1_68_s_17	15950537	Thus, arachidonic acid, the product  of PLA2, induces SM hydrolysis   [16], the cytosolic PLA2 can be inhibited by sphingosine   [17] and by SM   [17] and   [18], the inhibition by SM can be removed by sphingomyelinase   [18], ceramide accelerates the translocation of calcium-dependent PLA2 from cytosol to membranes in platelets   [19], and sphingosine and sphinganine directly inhibit PLA2  [20].	transcription
69541	11	336196	5	NULL	NULL	0	NULL	sphingosine	Chemical		inhibits		directly			PLA2	GP				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1735_1_68_s_17	15950537	Thus, arachidonic acid, the product  of PLA2, induces SM hydrolysis   [16], the cytosolic PLA2 can be inhibited by sphingosine   [17] and by SM   [17] and   [18], the inhibition by SM can be removed by sphingomyelinase   [18], ceramide accelerates the translocation of calcium-dependent PLA2 from cytosol to membranes in platelets   [19], and sphingosine and sphinganine directly inhibit PLA2  [20].	transcription
69542	12	336196	5	NULL	NULL	0	NULL	sphinganine	Chemical		inhibits		directly			PLA2	GP				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1735_1_68_s_17	15950537	Thus, arachidonic acid, the product  of PLA2, induces SM hydrolysis   [16], the cytosolic PLA2 can be inhibited by sphingosine   [17] and by SM   [17] and   [18], the inhibition by SM can be removed by sphingomyelinase   [18], ceramide accelerates the translocation of calcium-dependent PLA2 from cytosol to membranes in platelets   [19], and sphingosine and sphinganine directly inhibit PLA2  [20].	transcription
71560	1	336196	7	NULL	NULL	0	NULL	arachidonic acid	Chemical		is the product of					PLA2	GP				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1735_1_68_s_17	15950537	Thus, arachidonic acid, the product  of PLA2, induces SM hydrolysis   [16], the cytosolic PLA2 can be inhibited by sphingosine   [17] and by SM   [17] and   [18], the inhibition by SM can be removed by sphingomyelinase   [18], ceramide accelerates the translocation of calcium-dependent PLA2 from cytosol to membranes in platelets   [19], and sphingosine and sphinganine directly inhibit PLA2  [20].	transcription
71561	2	336196	7	NULL	NULL	0	NULL	arachidonic acid	Chemical		induces					SM	Chemical	hydrolysis of			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1735_1_68_s_17	15950537	Thus, arachidonic acid, the product  of PLA2, induces SM hydrolysis   [16], the cytosolic PLA2 can be inhibited by sphingosine   [17] and by SM   [17] and   [18], the inhibition by SM can be removed by sphingomyelinase   [18], ceramide accelerates the translocation of calcium-dependent PLA2 from cytosol to membranes in platelets   [19], and sphingosine and sphinganine directly inhibit PLA2  [20].	transcription
71562	3	336196	7	NULL	NULL	0	NULL	sphingosine	Chemical		inhibit					PLA2	GP	cytosolic			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1735_1_68_s_17	15950537	Thus, arachidonic acid, the product  of PLA2, induces SM hydrolysis   [16], the cytosolic PLA2 can be inhibited by sphingosine   [17] and by SM   [17] and   [18], the inhibition by SM can be removed by sphingomyelinase   [18], ceramide accelerates the translocation of calcium-dependent PLA2 from cytosol to membranes in platelets   [19], and sphingosine and sphinganine directly inhibit PLA2  [20].	transcription
71563	4	336196	7	NULL	NULL	0	NULL	SM	Chemical		inhibit					PLA2	GP	cytosolic			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1735_1_68_s_17	15950537	Thus, arachidonic acid, the product  of PLA2, induces SM hydrolysis   [16], the cytosolic PLA2 can be inhibited by sphingosine   [17] and by SM   [17] and   [18], the inhibition by SM can be removed by sphingomyelinase   [18], ceramide accelerates the translocation of calcium-dependent PLA2 from cytosol to membranes in platelets   [19], and sphingosine and sphinganine directly inhibit PLA2  [20].	transcription
71564	5	336196	7	NULL	NULL	0	NULL	sphingomyelinase	GP		remove					statement 4	Process	inhibition of			NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1735_1_68_s_17	15950537	Thus, arachidonic acid, the product  of PLA2, induces SM hydrolysis   [16], the cytosolic PLA2 can be inhibited by sphingosine   [17] and by SM   [17] and   [18], the inhibition by SM can be removed by sphingomyelinase   [18], ceramide accelerates the translocation of calcium-dependent PLA2 from cytosol to membranes in platelets   [19], and sphingosine and sphinganine directly inhibit PLA2  [20].	transcription
71565	6	336196	7	NULL	NULL	0	NULL	 PLA2	GP	calcium-dependent	translocated from					cytosol	CellComponent				NULL	platelets	0	NULL	NULL	NULL	gw70_biochimbiophysacta_1735_1_68_s_17	15950537	Thus, arachidonic acid, the product  of PLA2, induces SM hydrolysis   [16], the cytosolic PLA2 can be inhibited by sphingosine   [17] and by SM   [17] and   [18], the inhibition by SM can be removed by sphingomyelinase   [18], ceramide accelerates the translocation of calcium-dependent PLA2 from cytosol to membranes in platelets   [19], and sphingosine and sphinganine directly inhibit PLA2  [20].	transcription
71566	7	336196	7	NULL	NULL	0	NULL	PLA2	GP	calcium-dependent	translocated to					membranes	CellComponent				NULL	platelets	0	NULL	NULL	NULL	gw70_biochimbiophysacta_1735_1_68_s_17	15950537	Thus, arachidonic acid, the product  of PLA2, induces SM hydrolysis   [16], the cytosolic PLA2 can be inhibited by sphingosine   [17] and by SM   [17] and   [18], the inhibition by SM can be removed by sphingomyelinase   [18], ceramide accelerates the translocation of calcium-dependent PLA2 from cytosol to membranes in platelets   [19], and sphingosine and sphinganine directly inhibit PLA2  [20].	transcription
71567	8	336196	7	NULL	NULL	0	NULL	statement 6	Process		occur along with					statement 7	Process				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1735_1_68_s_17	15950537	Thus, arachidonic acid, the product  of PLA2, induces SM hydrolysis   [16], the cytosolic PLA2 can be inhibited by sphingosine   [17] and by SM   [17] and   [18], the inhibition by SM can be removed by sphingomyelinase   [18], ceramide accelerates the translocation of calcium-dependent PLA2 from cytosol to membranes in platelets   [19], and sphingosine and sphinganine directly inhibit PLA2  [20].	transcription
71568	9	336196	7	NULL	NULL	0	NULL	ceramide	Chemical		accelerates					statement 8	Process				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1735_1_68_s_17	15950537	Thus, arachidonic acid, the product  of PLA2, induces SM hydrolysis   [16], the cytosolic PLA2 can be inhibited by sphingosine   [17] and by SM   [17] and   [18], the inhibition by SM can be removed by sphingomyelinase   [18], ceramide accelerates the translocation of calcium-dependent PLA2 from cytosol to membranes in platelets   [19], and sphingosine and sphinganine directly inhibit PLA2  [20].	transcription
71569	10	336196	7	NULL	NULL	0	NULL	sphingosine	Chemical		inhibit		directly			PLA2	GP				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1735_1_68_s_17	15950537	Thus, arachidonic acid, the product  of PLA2, induces SM hydrolysis   [16], the cytosolic PLA2 can be inhibited by sphingosine   [17] and by SM   [17] and   [18], the inhibition by SM can be removed by sphingomyelinase   [18], ceramide accelerates the translocation of calcium-dependent PLA2 from cytosol to membranes in platelets   [19], and sphingosine and sphinganine directly inhibit PLA2  [20].	transcription
71570	11	336196	7	NULL	NULL	0	NULL	sphinganine	Chemical		inhibit		directly			PLA2	GP				NULL		0	NULL	NULL	NULL	gw70_biochimbiophysacta_1735_1_68_s_17	15950537	Thus, arachidonic acid, the product  of PLA2, induces SM hydrolysis   [16], the cytosolic PLA2 can be inhibited by sphingosine   [17] and by SM   [17] and   [18], the inhibition by SM can be removed by sphingomyelinase   [18], ceramide accelerates the translocation of calcium-dependent PLA2 from cytosol to membranes in platelets   [19], and sphingosine and sphinganine directly inhibit PLA2  [20].	transcription
69543	1	336197	5	NULL	NULL	0	NULL	PI-3K	GP	activation of	is induced by					oxLDL	Chemical				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1990_s_5	12482824	Methods and Results --  Coimmunoprecipitation experiments and the use of inhibitors and dominant-negative mutant showed that oxLDL-induced PI-3K activation is dependent on EGFR. PI-3K activation is independent of the sphingomyelin/ceramide/sphingosine-1-phosphate pathway, because PI-3K inhibition by LY294002 or dominant-negative deltap85 mutant does not abrogate sphingomyelin hydrolysis, and, conversely, the use of permeant C2-ceramide and of  N,N-dimethyl-sphingosine, a sphingosine kinase inhibitor, does not alter PI-3K activity.	transcription
69544	2	336197	5	NULL	NULL	0	NULL	statement 1	Process		is dependent on					EGFR	GP				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1990_s_5	12482824	Methods and Results --  Coimmunoprecipitation experiments and the use of inhibitors and dominant-negative mutant showed that oxLDL-induced PI-3K activation is dependent on EGFR. PI-3K activation is independent of the sphingomyelin/ceramide/sphingosine-1-phosphate pathway, because PI-3K inhibition by LY294002 or dominant-negative deltap85 mutant does not abrogate sphingomyelin hydrolysis, and, conversely, the use of permeant C2-ceramide and of  N,N-dimethyl-sphingosine, a sphingosine kinase inhibitor, does not alter PI-3K activity.	transcription
69545	3	336197	5	NULL	NULL	0	NULL	PI-3K	GP	activation of	is independent of					sphingomyelin/ceramide/sphingosine-1-phosphate pathway	Process				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1990_s_5	12482824	Methods and Results --  Coimmunoprecipitation experiments and the use of inhibitors and dominant-negative mutant showed that oxLDL-induced PI-3K activation is dependent on EGFR. PI-3K activation is independent of the sphingomyelin/ceramide/sphingosine-1-phosphate pathway, because PI-3K inhibition by LY294002 or dominant-negative deltap85 mutant does not abrogate sphingomyelin hydrolysis, and, conversely, the use of permeant C2-ceramide and of  N,N-dimethyl-sphingosine, a sphingosine kinase inhibitor, does not alter PI-3K activity.	transcription
69546	4	336197	5	NULL	NULL	0	NULL	PI-3K	GP		is inhibited by					LY294002	Chemical				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1990_s_5	12482824	Methods and Results --  Coimmunoprecipitation experiments and the use of inhibitors and dominant-negative mutant showed that oxLDL-induced PI-3K activation is dependent on EGFR. PI-3K activation is independent of the sphingomyelin/ceramide/sphingosine-1-phosphate pathway, because PI-3K inhibition by LY294002 or dominant-negative deltap85 mutant does not abrogate sphingomyelin hydrolysis, and, conversely, the use of permeant C2-ceramide and of  N,N-dimethyl-sphingosine, a sphingosine kinase inhibitor, does not alter PI-3K activity.	transcription
69547	5	336197	5	NULL	NULL	0	NULL	PI-3K	GP		is inhibited by					deltap85	GP	dominant-negative mutant			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1990_s_5	12482824	Methods and Results --  Coimmunoprecipitation experiments and the use of inhibitors and dominant-negative mutant showed that oxLDL-induced PI-3K activation is dependent on EGFR. PI-3K activation is independent of the sphingomyelin/ceramide/sphingosine-1-phosphate pathway, because PI-3K inhibition by LY294002 or dominant-negative deltap85 mutant does not abrogate sphingomyelin hydrolysis, and, conversely, the use of permeant C2-ceramide and of  N,N-dimethyl-sphingosine, a sphingosine kinase inhibitor, does not alter PI-3K activity.	transcription
69548	6	336197	5	NULL	NULL	0	NULL	statement 4	Process		doe not abrogate					sphingomyelin	Chemical	hydrolysis of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1990_s_5	12482824	Methods and Results --  Coimmunoprecipitation experiments and the use of inhibitors and dominant-negative mutant showed that oxLDL-induced PI-3K activation is dependent on EGFR. PI-3K activation is independent of the sphingomyelin/ceramide/sphingosine-1-phosphate pathway, because PI-3K inhibition by LY294002 or dominant-negative deltap85 mutant does not abrogate sphingomyelin hydrolysis, and, conversely, the use of permeant C2-ceramide and of  N,N-dimethyl-sphingosine, a sphingosine kinase inhibitor, does not alter PI-3K activity.	transcription
69549	7	336197	5	NULL	NULL	0	NULL	statement 5	Process		doe not abrogate					sphingomyelin	Chemical	hydrolysis of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1990_s_5	12482824	Methods and Results --  Coimmunoprecipitation experiments and the use of inhibitors and dominant-negative mutant showed that oxLDL-induced PI-3K activation is dependent on EGFR. PI-3K activation is independent of the sphingomyelin/ceramide/sphingosine-1-phosphate pathway, because PI-3K inhibition by LY294002 or dominant-negative deltap85 mutant does not abrogate sphingomyelin hydrolysis, and, conversely, the use of permeant C2-ceramide and of  N,N-dimethyl-sphingosine, a sphingosine kinase inhibitor, does not alter PI-3K activity.	transcription
69550	8	336197	5	NULL	NULL	0	NULL	C2-ceramide	Chemical	permeant	does not alter					PI-3K	GP	activity of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1990_s_5	12482824	Methods and Results --  Coimmunoprecipitation experiments and the use of inhibitors and dominant-negative mutant showed that oxLDL-induced PI-3K activation is dependent on EGFR. PI-3K activation is independent of the sphingomyelin/ceramide/sphingosine-1-phosphate pathway, because PI-3K inhibition by LY294002 or dominant-negative deltap85 mutant does not abrogate sphingomyelin hydrolysis, and, conversely, the use of permeant C2-ceramide and of  N,N-dimethyl-sphingosine, a sphingosine kinase inhibitor, does not alter PI-3K activity.	transcription
69551	9	336197	5	NULL	NULL	0	NULL	N,N-dimethyl-sphingosine	Chemical		does not alter					PI-3K	GP	activity of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1990_s_5	12482824	Methods and Results --  Coimmunoprecipitation experiments and the use of inhibitors and dominant-negative mutant showed that oxLDL-induced PI-3K activation is dependent on EGFR. PI-3K activation is independent of the sphingomyelin/ceramide/sphingosine-1-phosphate pathway, because PI-3K inhibition by LY294002 or dominant-negative deltap85 mutant does not abrogate sphingomyelin hydrolysis, and, conversely, the use of permeant C2-ceramide and of  N,N-dimethyl-sphingosine, a sphingosine kinase inhibitor, does not alter PI-3K activity.	transcription
69552	10	336197	5	NULL	NULL	0	NULL	N,N-dimethyl-sphingosine	Chemical		is an inhibitor of					sphingosine kinase	GP				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1990_s_5	12482824	Methods and Results --  Coimmunoprecipitation experiments and the use of inhibitors and dominant-negative mutant showed that oxLDL-induced PI-3K activation is dependent on EGFR. PI-3K activation is independent of the sphingomyelin/ceramide/sphingosine-1-phosphate pathway, because PI-3K inhibition by LY294002 or dominant-negative deltap85 mutant does not abrogate sphingomyelin hydrolysis, and, conversely, the use of permeant C2-ceramide and of  N,N-dimethyl-sphingosine, a sphingosine kinase inhibitor, does not alter PI-3K activity.	transcription
71571	1	336197	7	NULL	NULL	0	NULL	oxLDL	Chemical		induce					PI-3K	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1990_s_5	12482824	Methods and Results --  Coimmunoprecipitation experiments and the use of inhibitors and dominant-negative mutant showed that oxLDL-induced PI-3K activation is dependent on EGFR. PI-3K activation is independent of the sphingomyelin/ceramide/sphingosine-1-phosphate pathway, because PI-3K inhibition by LY294002 or dominant-negative deltap85 mutant does not abrogate sphingomyelin hydrolysis, and, conversely, the use of permeant C2-ceramide and of  N,N-dimethyl-sphingosine, a sphingosine kinase inhibitor, does not alter PI-3K activity.	transcription
71572	2	336197	7	NULL	NULL	0	NULL	statement 1	Process		depends on					EGFR	GP				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1990_s_5	12482824	Methods and Results --  Coimmunoprecipitation experiments and the use of inhibitors and dominant-negative mutant showed that oxLDL-induced PI-3K activation is dependent on EGFR. PI-3K activation is independent of the sphingomyelin/ceramide/sphingosine-1-phosphate pathway, because PI-3K inhibition by LY294002 or dominant-negative deltap85 mutant does not abrogate sphingomyelin hydrolysis, and, conversely, the use of permeant C2-ceramide and of  N,N-dimethyl-sphingosine, a sphingosine kinase inhibitor, does not alter PI-3K activity.	transcription
71573	3	336197	7	NULL	NULL	0	NULL	PI-3K	GP	activation of	is independent of					sphingomyelin pathway	Process				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1990_s_5	12482824	Methods and Results --  Coimmunoprecipitation experiments and the use of inhibitors and dominant-negative mutant showed that oxLDL-induced PI-3K activation is dependent on EGFR. PI-3K activation is independent of the sphingomyelin/ceramide/sphingosine-1-phosphate pathway, because PI-3K inhibition by LY294002 or dominant-negative deltap85 mutant does not abrogate sphingomyelin hydrolysis, and, conversely, the use of permeant C2-ceramide and of  N,N-dimethyl-sphingosine, a sphingosine kinase inhibitor, does not alter PI-3K activity.	transcription
71575	4	336197	7	NULL	NULL	NULL	NULL	PI-3K	GP	activation of	is independent of					ceramide pathway	Process				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1990_s_5	12482824	Methods and Results --  Coimmunoprecipitation experiments and the use of inhibitors and dominant-negative mutant showed that oxLDL-induced PI-3K activation is dependent on EGFR. PI-3K activation is independent of the sphingomyelin/ceramide/sphingosine-1-phosphate pathway, because PI-3K inhibition by LY294002 or dominant-negative deltap85 mutant does not abrogate sphingomyelin hydrolysis, and, conversely, the use of permeant C2-ceramide and of  N,N-dimethyl-sphingosine, a sphingosine kinase inhibitor, does not alter PI-3K activity.	transcription
71576	5	336197	7	NULL	NULL	0	NULL	PI-3K	GP	activation of	is independent of					sphingosine-1-phosphate pathway	Process				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1990_s_5	12482824	Methods and Results --  Coimmunoprecipitation experiments and the use of inhibitors and dominant-negative mutant showed that oxLDL-induced PI-3K activation is dependent on EGFR. PI-3K activation is independent of the sphingomyelin/ceramide/sphingosine-1-phosphate pathway, because PI-3K inhibition by LY294002 or dominant-negative deltap85 mutant does not abrogate sphingomyelin hydrolysis, and, conversely, the use of permeant C2-ceramide and of  N,N-dimethyl-sphingosine, a sphingosine kinase inhibitor, does not alter PI-3K activity.	transcription
71577	6	336197	7	NULL	NULL	0	NULL	LY294002	Chemical		inhibit					PI-3K	GP				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1990_s_5	12482824	Methods and Results --  Coimmunoprecipitation experiments and the use of inhibitors and dominant-negative mutant showed that oxLDL-induced PI-3K activation is dependent on EGFR. PI-3K activation is independent of the sphingomyelin/ceramide/sphingosine-1-phosphate pathway, because PI-3K inhibition by LY294002 or dominant-negative deltap85 mutant does not abrogate sphingomyelin hydrolysis, and, conversely, the use of permeant C2-ceramide and of  N,N-dimethyl-sphingosine, a sphingosine kinase inhibitor, does not alter PI-3K activity.	transcription
71578	7	336197	7	NULL	NULL	NULL	NULL	deltap85	GP	dominant-negative mutant	inhibit					PI 3-K	GP				NULL		NULL	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1990_s_5	12482824	Methods and Results --  Coimmunoprecipitation experiments and the use of inhibitors and dominant-negative mutant showed that oxLDL-induced PI-3K activation is dependent on EGFR. PI-3K activation is independent of the sphingomyelin/ceramide/sphingosine-1-phosphate pathway, because PI-3K inhibition by LY294002 or dominant-negative deltap85 mutant does not abrogate sphingomyelin hydrolysis, and, conversely, the use of permeant C2-ceramide and of  N,N-dimethyl-sphingosine, a sphingosine kinase inhibitor, does not alter PI-3K activity.	transcription
71579	8	336197	7	NULL	NULL	0	NULL	statement 6	Process		does not abrogate					sphingomyelin	Chemical	hydrolysis of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1990_s_5	12482824	Methods and Results --  Coimmunoprecipitation experiments and the use of inhibitors and dominant-negative mutant showed that oxLDL-induced PI-3K activation is dependent on EGFR. PI-3K activation is independent of the sphingomyelin/ceramide/sphingosine-1-phosphate pathway, because PI-3K inhibition by LY294002 or dominant-negative deltap85 mutant does not abrogate sphingomyelin hydrolysis, and, conversely, the use of permeant C2-ceramide and of  N,N-dimethyl-sphingosine, a sphingosine kinase inhibitor, does not alter PI-3K activity.	transcription
71580	9	336197	7	NULL	NULL	0	NULL	statement 7	Process		does not abrogate					sphingomyelin	Chemical	hydrolysis of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1990_s_5	12482824	Methods and Results --  Coimmunoprecipitation experiments and the use of inhibitors and dominant-negative mutant showed that oxLDL-induced PI-3K activation is dependent on EGFR. PI-3K activation is independent of the sphingomyelin/ceramide/sphingosine-1-phosphate pathway, because PI-3K inhibition by LY294002 or dominant-negative deltap85 mutant does not abrogate sphingomyelin hydrolysis, and, conversely, the use of permeant C2-ceramide and of  N,N-dimethyl-sphingosine, a sphingosine kinase inhibitor, does not alter PI-3K activity.	transcription
71581	10	336197	7	NULL	NULL	0	NULL	statement 6	Process		is an alternative to					statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1990_s_5	12482824	Methods and Results --  Coimmunoprecipitation experiments and the use of inhibitors and dominant-negative mutant showed that oxLDL-induced PI-3K activation is dependent on EGFR. PI-3K activation is independent of the sphingomyelin/ceramide/sphingosine-1-phosphate pathway, because PI-3K inhibition by LY294002 or dominant-negative deltap85 mutant does not abrogate sphingomyelin hydrolysis, and, conversely, the use of permeant C2-ceramide and of  N,N-dimethyl-sphingosine, a sphingosine kinase inhibitor, does not alter PI-3K activity.	transcription
71582	11	336197	7	NULL	NULL	0	NULL	C2-ceramide	Chemical		does not alter					PI-3K 	GP	activity of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1990_s_5	12482824	Methods and Results --  Coimmunoprecipitation experiments and the use of inhibitors and dominant-negative mutant showed that oxLDL-induced PI-3K activation is dependent on EGFR. PI-3K activation is independent of the sphingomyelin/ceramide/sphingosine-1-phosphate pathway, because PI-3K inhibition by LY294002 or dominant-negative deltap85 mutant does not abrogate sphingomyelin hydrolysis, and, conversely, the use of permeant C2-ceramide and of  N,N-dimethyl-sphingosine, a sphingosine kinase inhibitor, does not alter PI-3K activity.	transcription
71583	12	336197	7	NULL	NULL	0	NULL	N,N-dimethyl-sphingosine	Chemical		does not alter					PI-3K 	GP	activity of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1990_s_5	12482824	Methods and Results --  Coimmunoprecipitation experiments and the use of inhibitors and dominant-negative mutant showed that oxLDL-induced PI-3K activation is dependent on EGFR. PI-3K activation is independent of the sphingomyelin/ceramide/sphingosine-1-phosphate pathway, because PI-3K inhibition by LY294002 or dominant-negative deltap85 mutant does not abrogate sphingomyelin hydrolysis, and, conversely, the use of permeant C2-ceramide and of  N,N-dimethyl-sphingosine, a sphingosine kinase inhibitor, does not alter PI-3K activity.	transcription
71584	13	336197	7	NULL	NULL	0	NULL	N,N-dimethyl-sphingosine	Chemical		inhibit					sphingosine kinase	GP				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_22_12_1990_s_5	12482824	Methods and Results --  Coimmunoprecipitation experiments and the use of inhibitors and dominant-negative mutant showed that oxLDL-induced PI-3K activation is dependent on EGFR. PI-3K activation is independent of the sphingomyelin/ceramide/sphingosine-1-phosphate pathway, because PI-3K inhibition by LY294002 or dominant-negative deltap85 mutant does not abrogate sphingomyelin hydrolysis, and, conversely, the use of permeant C2-ceramide and of  N,N-dimethyl-sphingosine, a sphingosine kinase inhibitor, does not alter PI-3K activity.	transcription
71585	1	336200	7	NULL	NULL	NULL	NULL	PDMP	Chemical		inhibits		potently			glucosylceramide synthase	GP	activity of			NULL	in vitro	NULL	NULL	NULL	NULL	gw60_cellbiol_158_6_1039_s_156	12235122	PDMP at 10 muM, a concentration that potently inhibits glucosylceramide synthase activity in vitro ( Shayman et al., 2000), increased ceramide by 2.5-fold over basal levels in untreated and dihydro-S1P - treated mSPP-1 - expressing cells, and markedly augmented the elevated ceramide accumulation induced by S1P ( Fig. 10 A) without significantly affecting sphingosine levels ( Fig. 10 B).	transcription
71586	2	336200	7	NULL	NULL	NULL	NULL	PDMP	Chemical		increase					ceramide	Chemical				NULL	untreated mSPP-1 - expressing cells	NULL	NULL	NULL	NULL	gw60_cellbiol_158_6_1039_s_156	12235122	PDMP at 10 muM, a concentration that potently inhibits glucosylceramide synthase activity in vitro ( Shayman et al., 2000), increased ceramide by 2.5-fold over basal levels in untreated and dihydro-S1P - treated mSPP-1 - expressing cells, and markedly augmented the elevated ceramide accumulation induced by S1P ( Fig. 10 A) without significantly affecting sphingosine levels ( Fig. 10 B).	transcription
71587	3	336200	7	NULL	NULL	0	NULL	PDMP	Chemical		increase					ceramide	Chemical				NULL	dihydro-S1P - treated mSPP-1 - expressing cells	0	NULL	NULL	NULL	gw60_cellbiol_158_6_1039_s_156	12235122	PDMP at 10 muM, a concentration that potently inhibits glucosylceramide synthase activity in vitro ( Shayman et al., 2000), increased ceramide by 2.5-fold over basal levels in untreated and dihydro-S1P - treated mSPP-1 - expressing cells, and markedly augmented the elevated ceramide accumulation induced by S1P ( Fig. 10 A) without significantly affecting sphingosine levels ( Fig. 10 B).	transcription
71588	4	336200	7	NULL	NULL	0	NULL	PDMP	Chemical		augments		markedly			ceramide	Chemical	elevated			NULL		0	NULL	NULL	NULL	gw60_cellbiol_158_6_1039_s_156	12235122	PDMP at 10 muM, a concentration that potently inhibits glucosylceramide synthase activity in vitro ( Shayman et al., 2000), increased ceramide by 2.5-fold over basal levels in untreated and dihydro-S1P - treated mSPP-1 - expressing cells, and markedly augmented the elevated ceramide accumulation induced by S1P ( Fig. 10 A) without significantly affecting sphingosine levels ( Fig. 10 B).	transcription
71589	5	336200	7	NULL	NULL	0	NULL	S1P	Chemical		induce					ceramide	Chemical	accumulation of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_158_6_1039_s_156	12235122	PDMP at 10 muM, a concentration that potently inhibits glucosylceramide synthase activity in vitro ( Shayman et al., 2000), increased ceramide by 2.5-fold over basal levels in untreated and dihydro-S1P - treated mSPP-1 - expressing cells, and markedly augmented the elevated ceramide accumulation induced by S1P ( Fig. 10 A) without significantly affecting sphingosine levels ( Fig. 10 B).	transcription
71590	6	336200	7	NULL	NULL	0	NULL	statement 4	Process		does not affect		significantly			sphingosine	Chemical	levels of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_158_6_1039_s_156	12235122	PDMP at 10 muM, a concentration that potently inhibits glucosylceramide synthase activity in vitro ( Shayman et al., 2000), increased ceramide by 2.5-fold over basal levels in untreated and dihydro-S1P - treated mSPP-1 - expressing cells, and markedly augmented the elevated ceramide accumulation induced by S1P ( Fig. 10 A) without significantly affecting sphingosine levels ( Fig. 10 B).	transcription
69554	1	336201	5	NULL	NULL	0	NULL	ceramide	Chemical	accumulation of	does not effect					6-([ N-(7-nitrobenzo-2-oxa-1,3-diazol-4-yl)amino]hexanoyl)-sphingosine	Chemical	trafficking of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_13_5055_s_6	16782891	In contrast, ceramide accumulation had no effect on either the trafficking or the metabolism of 6-([ N-(7-nitrobenzo-2-oxa-1,3-diazol-4-yl)amino]hexanoyl)-sphingosine, which rapidly labels the Golgi even at 4 degrees C. Protein trafficking from the ER to the Golgi, determined with vesicular stomatitis virus ts045 G protein fused to green fluorescent protein, was also inhibited in SPP-1-overexpressing cells in the presence of S1P but not in the presence of dihydro-S1P.	transcription
69555	2	336201	5	NULL	NULL	0	NULL	ceramide	Chemical	accumulation of	does not effect					6-([ N-(7-nitrobenzo-2-oxa-1,3-diazol-4-yl)amino]hexanoyl)-sphingosine	Chemical	metabolism of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_13_5055_s_6	16782891	In contrast, ceramide accumulation had no effect on either the trafficking or the metabolism of 6-([ N-(7-nitrobenzo-2-oxa-1,3-diazol-4-yl)amino]hexanoyl)-sphingosine, which rapidly labels the Golgi even at 4 degrees C. Protein trafficking from the ER to the Golgi, determined with vesicular stomatitis virus ts045 G protein fused to green fluorescent protein, was also inhibited in SPP-1-overexpressing cells in the presence of S1P but not in the presence of dihydro-S1P.	transcription
69556	3	336201	5	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_13_5055_s_6	16782891	In contrast, ceramide accumulation had no effect on either the trafficking or the metabolism of 6-([ N-(7-nitrobenzo-2-oxa-1,3-diazol-4-yl)amino]hexanoyl)-sphingosine, which rapidly labels the Golgi even at 4 degrees C. Protein trafficking from the ER to the Golgi, determined with vesicular stomatitis virus ts045 G protein fused to green fluorescent protein, was also inhibited in SPP-1-overexpressing cells in the presence of S1P but not in the presence of dihydro-S1P.	transcription
69557	4	336201	5	NULL	NULL	0	NULL	6-([ N-(7-nitrobenzo-2-oxa-1,3-diazol-4-yl)amino]hexanoyl)-sphingosine	Chemical		labels		rapidly			Golgi	CellComponent				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_13_5055_s_6	16782891	In contrast, ceramide accumulation had no effect on either the trafficking or the metabolism of 6-([ N-(7-nitrobenzo-2-oxa-1,3-diazol-4-yl)amino]hexanoyl)-sphingosine, which rapidly labels the Golgi even at 4 degrees C. Protein trafficking from the ER to the Golgi, determined with vesicular stomatitis virus ts045 G protein fused to green fluorescent protein, was also inhibited in SPP-1-overexpressing cells in the presence of S1P but not in the presence of dihydro-S1P.	transcription
69559	5	336201	5	NULL	NULL	0	NULL	ts045 G protein	GP	vesicular stomatitis virus	is fused to					green fluorescent protein	GP				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_13_5055_s_6	16782891	In contrast, ceramide accumulation had no effect on either the trafficking or the metabolism of 6-([ N-(7-nitrobenzo-2-oxa-1,3-diazol-4-yl)amino]hexanoyl)-sphingosine, which rapidly labels the Golgi even at 4 degrees C. Protein trafficking from the ER to the Golgi, determined with vesicular stomatitis virus ts045 G protein fused to green fluorescent protein, was also inhibited in SPP-1-overexpressing cells in the presence of S1P but not in the presence of dihydro-S1P.	transcription
69560	6	336201	5	NULL	NULL	NULL	NULL	statement 5	GP		trafficked from					ER	CellComponent				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_26_13_5055_s_6	16782891	In contrast, ceramide accumulation had no effect on either the trafficking or the metabolism of 6-([ N-(7-nitrobenzo-2-oxa-1,3-diazol-4-yl)amino]hexanoyl)-sphingosine, which rapidly labels the Golgi even at 4 degrees C. Protein trafficking from the ER to the Golgi, determined with vesicular stomatitis virus ts045 G protein fused to green fluorescent protein, was also inhibited in SPP-1-overexpressing cells in the presence of S1P but not in the presence of dihydro-S1P.	transcription
69561	7	336201	5	NULL	NULL	0	NULL	statement 5	GP		trafficked to					Golgi	CellComponent				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_13_5055_s_6	16782891	In contrast, ceramide accumulation had no effect on either the trafficking or the metabolism of 6-([ N-(7-nitrobenzo-2-oxa-1,3-diazol-4-yl)amino]hexanoyl)-sphingosine, which rapidly labels the Golgi even at 4 degrees C. Protein trafficking from the ER to the Golgi, determined with vesicular stomatitis virus ts045 G protein fused to green fluorescent protein, was also inhibited in SPP-1-overexpressing cells in the presence of S1P but not in the presence of dihydro-S1P.	transcription
69562	8	336201	5	NULL	NULL	0	NULL	statement 6	Process		occurs along with					statement 7	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_13_5055_s_6	16782891	In contrast, ceramide accumulation had no effect on either the trafficking or the metabolism of 6-([ N-(7-nitrobenzo-2-oxa-1,3-diazol-4-yl)amino]hexanoyl)-sphingosine, which rapidly labels the Golgi even at 4 degrees C. Protein trafficking from the ER to the Golgi, determined with vesicular stomatitis virus ts045 G protein fused to green fluorescent protein, was also inhibited in SPP-1-overexpressing cells in the presence of S1P but not in the presence of dihydro-S1P.	transcription
69563	9	336201	5	NULL	NULL	0	NULL	statement 6	Process		is inhibited in					S1P	Chemical	presence of			NULL	SPP-1-overexpressing cells	0	NULL	NULL	NULL	gw70_molcellbiol_26_13_5055_s_6	16782891	In contrast, ceramide accumulation had no effect on either the trafficking or the metabolism of 6-([ N-(7-nitrobenzo-2-oxa-1,3-diazol-4-yl)amino]hexanoyl)-sphingosine, which rapidly labels the Golgi even at 4 degrees C. Protein trafficking from the ER to the Golgi, determined with vesicular stomatitis virus ts045 G protein fused to green fluorescent protein, was also inhibited in SPP-1-overexpressing cells in the presence of S1P but not in the presence of dihydro-S1P.	transcription
69564	10	336201	5	NULL	NULL	0	NULL	statement 7	Process		is inhibited in					S1P	Chemical	presence of			NULL	SPP-1-overexpressing cells	0	NULL	NULL	NULL	gw70_molcellbiol_26_13_5055_s_6	16782891	In contrast, ceramide accumulation had no effect on either the trafficking or the metabolism of 6-([ N-(7-nitrobenzo-2-oxa-1,3-diazol-4-yl)amino]hexanoyl)-sphingosine, which rapidly labels the Golgi even at 4 degrees C. Protein trafficking from the ER to the Golgi, determined with vesicular stomatitis virus ts045 G protein fused to green fluorescent protein, was also inhibited in SPP-1-overexpressing cells in the presence of S1P but not in the presence of dihydro-S1P.	transcription
69565	12	336201	5	NULL	NULL	NULL	NULL	statement 7	Process		is not inhibited in					dihydro-S1P	Chemical	presence of			NULL	SPP-1-overexpressing cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_13_5055_s_6	16782891	In contrast, ceramide accumulation had no effect on either the trafficking or the metabolism of 6-([ N-(7-nitrobenzo-2-oxa-1,3-diazol-4-yl)amino]hexanoyl)-sphingosine, which rapidly labels the Golgi even at 4 degrees C. Protein trafficking from the ER to the Golgi, determined with vesicular stomatitis virus ts045 G protein fused to green fluorescent protein, was also inhibited in SPP-1-overexpressing cells in the presence of S1P but not in the presence of dihydro-S1P.	transcription
69566	11	336201	5	NULL	NULL	NULL	NULL	statement 6	Process		is not inhibited in					dihydro-S1P	Chemical	presence of			NULL	SPP-1-overexpressing cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_13_5055_s_6	16782891	In contrast, ceramide accumulation had no effect on either the trafficking or the metabolism of 6-([ N-(7-nitrobenzo-2-oxa-1,3-diazol-4-yl)amino]hexanoyl)-sphingosine, which rapidly labels the Golgi even at 4 degrees C. Protein trafficking from the ER to the Golgi, determined with vesicular stomatitis virus ts045 G protein fused to green fluorescent protein, was also inhibited in SPP-1-overexpressing cells in the presence of S1P but not in the presence of dihydro-S1P.	transcription
71591	1	336201	7	NULL	NULL	0	NULL	ceramide 	Chemical	accumulation of	no effect on					 6-([ N-(7-nitrobenzo-2-oxa-1,3-diazol-4-yl)amino]hexanoyl)-sphingosine	Chemical	trafficking of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_13_5055_s_6	16782891	In contrast, ceramide accumulation had no effect on either the trafficking or the metabolism of 6-([ N-(7-nitrobenzo-2-oxa-1,3-diazol-4-yl)amino]hexanoyl)-sphingosine, which rapidly labels the Golgi even at 4 degrees C. Protein trafficking from the ER to the Golgi, determined with vesicular stomatitis virus ts045 G protein fused to green fluorescent protein, was also inhibited in SPP-1-overexpressing cells in the presence of S1P but not in the presence of dihydro-S1P.	transcription
71592	2	336201	7	NULL	NULL	0	NULL	ceramide	Chemical	accumulation of	no effect on					 6-([ N-(7-nitrobenzo-2-oxa-1,3-diazol-4-yl)amino]hexanoyl)-sphingosine	Chemical	metabolism of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_13_5055_s_6	16782891	In contrast, ceramide accumulation had no effect on either the trafficking or the metabolism of 6-([ N-(7-nitrobenzo-2-oxa-1,3-diazol-4-yl)amino]hexanoyl)-sphingosine, which rapidly labels the Golgi even at 4 degrees C. Protein trafficking from the ER to the Golgi, determined with vesicular stomatitis virus ts045 G protein fused to green fluorescent protein, was also inhibited in SPP-1-overexpressing cells in the presence of S1P but not in the presence of dihydro-S1P.	transcription
71593	3	336201	7	NULL	NULL	0	NULL	 6-([ N-(7-nitrobenzo-2-oxa-1,3-diazol-4-yl)amino]hexanoyl)-sphingosine	Chemical		labels		rapidly			Golgi	CellComponent				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_13_5055_s_6	16782891	In contrast, ceramide accumulation had no effect on either the trafficking or the metabolism of 6-([ N-(7-nitrobenzo-2-oxa-1,3-diazol-4-yl)amino]hexanoyl)-sphingosine, which rapidly labels the Golgi even at 4 degrees C. Protein trafficking from the ER to the Golgi, determined with vesicular stomatitis virus ts045 G protein fused to green fluorescent protein, was also inhibited in SPP-1-overexpressing cells in the presence of S1P but not in the presence of dihydro-S1P.	transcription
71594	4	336201	7	NULL	NULL	0	NULL	protein	GP		trafficking from					ER	CellComponent				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_13_5055_s_6	16782891	In contrast, ceramide accumulation had no effect on either the trafficking or the metabolism of 6-([ N-(7-nitrobenzo-2-oxa-1,3-diazol-4-yl)amino]hexanoyl)-sphingosine, which rapidly labels the Golgi even at 4 degrees C. Protein trafficking from the ER to the Golgi, determined with vesicular stomatitis virus ts045 G protein fused to green fluorescent protein, was also inhibited in SPP-1-overexpressing cells in the presence of S1P but not in the presence of dihydro-S1P.	transcription
71595	5	336201	7	NULL	NULL	0	NULL	Protein	GP		trafficking to					Golgi	CellComponent				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_13_5055_s_6	16782891	In contrast, ceramide accumulation had no effect on either the trafficking or the metabolism of 6-([ N-(7-nitrobenzo-2-oxa-1,3-diazol-4-yl)amino]hexanoyl)-sphingosine, which rapidly labels the Golgi even at 4 degrees C. Protein trafficking from the ER to the Golgi, determined with vesicular stomatitis virus ts045 G protein fused to green fluorescent protein, was also inhibited in SPP-1-overexpressing cells in the presence of S1P but not in the presence of dihydro-S1P.	transcription
71596	6	336201	7	NULL	NULL	0	NULL	statement 4	Process		occur along with					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_13_5055_s_6	16782891	In contrast, ceramide accumulation had no effect on either the trafficking or the metabolism of 6-([ N-(7-nitrobenzo-2-oxa-1,3-diazol-4-yl)amino]hexanoyl)-sphingosine, which rapidly labels the Golgi even at 4 degrees C. Protein trafficking from the ER to the Golgi, determined with vesicular stomatitis virus ts045 G protein fused to green fluorescent protein, was also inhibited in SPP-1-overexpressing cells in the presence of S1P but not in the presence of dihydro-S1P.	transcription
71597	7	336201	7	NULL	NULL	NULL	NULL	statement 6	Process		inhibited					S1P	Chemical	in the presence of			NULL	SPP-1-overexpressing cells	NULL	NULL	NULL	NULL	gw70_molcellbiol_26_13_5055_s_6	16782891	In contrast, ceramide accumulation had no effect on either the trafficking or the metabolism of 6-([ N-(7-nitrobenzo-2-oxa-1,3-diazol-4-yl)amino]hexanoyl)-sphingosine, which rapidly labels the Golgi even at 4 degrees C. Protein trafficking from the ER to the Golgi, determined with vesicular stomatitis virus ts045 G protein fused to green fluorescent protein, was also inhibited in SPP-1-overexpressing cells in the presence of S1P but not in the presence of dihydro-S1P.	transcription
71598	8	336201	7	NULL	NULL	0	NULL	statement 6	Process		is not inhibited					dihydro-S1P	Chemical	in the presence of			NULL	SPP-1-overexpressing cells	0	NULL	NULL	NULL	gw70_molcellbiol_26_13_5055_s_6	16782891	In contrast, ceramide accumulation had no effect on either the trafficking or the metabolism of 6-([ N-(7-nitrobenzo-2-oxa-1,3-diazol-4-yl)amino]hexanoyl)-sphingosine, which rapidly labels the Golgi even at 4 degrees C. Protein trafficking from the ER to the Golgi, determined with vesicular stomatitis virus ts045 G protein fused to green fluorescent protein, was also inhibited in SPP-1-overexpressing cells in the presence of S1P but not in the presence of dihydro-S1P.	transcription
69567	1	336202	5	NULL	NULL	0	NULL	Ca2+ transient	Process		is induced by					sphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_220	9915989	Nonetheless, although sphingosine-induced Ca2+ transients have been previously reported to occur via mobilization of Ca2+ from intracellular stores [ 33,  34], this study represents the first demonstration that ceramide regulates [Ca2+]i. Cch-induced Ca2+ transients occur via IP3-mediated mobilization of Ca2+ from intracellular stores and/or transmembrane influx of Ca2+ [ 22,  24].	transcription
69568	2	336202	5	NULL	NULL	0	NULL	Ca2+	Chemical		is mobilized from					intracellular stores	CellComponent				NULL		0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_220	9915989	Nonetheless, although sphingosine-induced Ca2+ transients have been previously reported to occur via mobilization of Ca2+ from intracellular stores [ 33,  34], this study represents the first demonstration that ceramide regulates [Ca2+]i. Cch-induced Ca2+ transients occur via IP3-mediated mobilization of Ca2+ from intracellular stores and/or transmembrane influx of Ca2+ [ 22,  24].	transcription
69569	3	336202	5	NULL	NULL	0	NULL	statement 1	Process		via					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_220	9915989	Nonetheless, although sphingosine-induced Ca2+ transients have been previously reported to occur via mobilization of Ca2+ from intracellular stores [ 33,  34], this study represents the first demonstration that ceramide regulates [Ca2+]i. Cch-induced Ca2+ transients occur via IP3-mediated mobilization of Ca2+ from intracellular stores and/or transmembrane influx of Ca2+ [ 22,  24].	transcription
69570	4	336202	5	NULL	NULL	0	NULL	ceramide	Chemical		regulates					[Ca2+]i	Chemical				NULL		0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_220	9915989	Nonetheless, although sphingosine-induced Ca2+ transients have been previously reported to occur via mobilization of Ca2+ from intracellular stores [ 33,  34], this study represents the first demonstration that ceramide regulates [Ca2+]i. Cch-induced Ca2+ transients occur via IP3-mediated mobilization of Ca2+ from intracellular stores and/or transmembrane influx of Ca2+ [ 22,  24].	transcription
69571	5	336202	5	NULL	NULL	0	NULL	Ca2+ transient	Process		is induced by					Cch	Chemical				NULL		0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_220	9915989	Nonetheless, although sphingosine-induced Ca2+ transients have been previously reported to occur via mobilization of Ca2+ from intracellular stores [ 33,  34], this study represents the first demonstration that ceramide regulates [Ca2+]i. Cch-induced Ca2+ transients occur via IP3-mediated mobilization of Ca2+ from intracellular stores and/or transmembrane influx of Ca2+ [ 22,  24].	transcription
69572	6	336202	5	NULL	NULL	0	NULL	IP3	Chemical		mediates					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_220	9915989	Nonetheless, although sphingosine-induced Ca2+ transients have been previously reported to occur via mobilization of Ca2+ from intracellular stores [ 33,  34], this study represents the first demonstration that ceramide regulates [Ca2+]i. Cch-induced Ca2+ transients occur via IP3-mediated mobilization of Ca2+ from intracellular stores and/or transmembrane influx of Ca2+ [ 22,  24].	transcription
69573	7	336202	5	NULL	NULL	0	NULL	statement 5	Process		via					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_220	9915989	Nonetheless, although sphingosine-induced Ca2+ transients have been previously reported to occur via mobilization of Ca2+ from intracellular stores [ 33,  34], this study represents the first demonstration that ceramide regulates [Ca2+]i. Cch-induced Ca2+ transients occur via IP3-mediated mobilization of Ca2+ from intracellular stores and/or transmembrane influx of Ca2+ [ 22,  24].	transcription
69574	8	336202	5	NULL	NULL	0	NULL	statement 5	Process		via					Ca2+	Chemical	transmembrane influx of			NULL		0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_220	9915989	Nonetheless, although sphingosine-induced Ca2+ transients have been previously reported to occur via mobilization of Ca2+ from intracellular stores [ 33,  34], this study represents the first demonstration that ceramide regulates [Ca2+]i. Cch-induced Ca2+ transients occur via IP3-mediated mobilization of Ca2+ from intracellular stores and/or transmembrane influx of Ca2+ [ 22,  24].	transcription
71599	1	336202	7	NULL	NULL	0	NULL	sphingosine	Chemical		induce					Ca2+	Chemical	transient			NULL		0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_220	9915989	Nonetheless, although sphingosine-induced Ca2+ transients have been previously reported to occur via mobilization of Ca2+ from intracellular stores [ 33,  34], this study represents the first demonstration that ceramide regulates [Ca2+]i. Cch-induced Ca2+ transients occur via IP3-mediated mobilization of Ca2+ from intracellular stores and/or transmembrane influx of Ca2+ [ 22,  24].	transcription
71600	2	336202	7	NULL	NULL	NULL	NULL	Ca2+	Chemical		mobilized from					intracellular stores	CellComponent				NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_220	9915989	Nonetheless, although sphingosine-induced Ca2+ transients have been previously reported to occur via mobilization of Ca2+ from intracellular stores [ 33,  34], this study represents the first demonstration that ceramide regulates [Ca2+]i. Cch-induced Ca2+ transients occur via IP3-mediated mobilization of Ca2+ from intracellular stores and/or transmembrane influx of Ca2+ [ 22,  24].	transcription
71601	3	336202	7	NULL	NULL	0	NULL	statement 1	Process		occur via					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_220	9915989	Nonetheless, although sphingosine-induced Ca2+ transients have been previously reported to occur via mobilization of Ca2+ from intracellular stores [ 33,  34], this study represents the first demonstration that ceramide regulates [Ca2+]i. Cch-induced Ca2+ transients occur via IP3-mediated mobilization of Ca2+ from intracellular stores and/or transmembrane influx of Ca2+ [ 22,  24].	transcription
71602	4	336202	7	NULL	NULL	0	NULL	ceramide	Chemical		regulates					[Ca2+]i	Chemical				NULL		0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_220	9915989	Nonetheless, although sphingosine-induced Ca2+ transients have been previously reported to occur via mobilization of Ca2+ from intracellular stores [ 33,  34], this study represents the first demonstration that ceramide regulates [Ca2+]i. Cch-induced Ca2+ transients occur via IP3-mediated mobilization of Ca2+ from intracellular stores and/or transmembrane influx of Ca2+ [ 22,  24].	transcription
71603	5	336202	7	NULL	NULL	0	NULL	Cch	Chemical		induce					Ca2+	Chemical	transient			NULL		0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_220	9915989	Nonetheless, although sphingosine-induced Ca2+ transients have been previously reported to occur via mobilization of Ca2+ from intracellular stores [ 33,  34], this study represents the first demonstration that ceramide regulates [Ca2+]i. Cch-induced Ca2+ transients occur via IP3-mediated mobilization of Ca2+ from intracellular stores and/or transmembrane influx of Ca2+ [ 22,  24].	transcription
71604	6	336202	7	NULL	NULL	0	NULL	IP3	Chemical		mediates					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_220	9915989	Nonetheless, although sphingosine-induced Ca2+ transients have been previously reported to occur via mobilization of Ca2+ from intracellular stores [ 33,  34], this study represents the first demonstration that ceramide regulates [Ca2+]i. Cch-induced Ca2+ transients occur via IP3-mediated mobilization of Ca2+ from intracellular stores and/or transmembrane influx of Ca2+ [ 22,  24].	transcription
71605	7	336202	7	NULL	NULL	0	NULL	statement 5	Process		occur via					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_220	9915989	Nonetheless, although sphingosine-induced Ca2+ transients have been previously reported to occur via mobilization of Ca2+ from intracellular stores [ 33,  34], this study represents the first demonstration that ceramide regulates [Ca2+]i. Cch-induced Ca2+ transients occur via IP3-mediated mobilization of Ca2+ from intracellular stores and/or transmembrane influx of Ca2+ [ 22,  24].	transcription
71606	8	336202	7	NULL	NULL	0	NULL	Ca2+	Chemical		mobilized from					Ca2+	Chemical	transmembrane influx of			NULL		0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_220	9915989	Nonetheless, although sphingosine-induced Ca2+ transients have been previously reported to occur via mobilization of Ca2+ from intracellular stores [ 33,  34], this study represents the first demonstration that ceramide regulates [Ca2+]i. Cch-induced Ca2+ transients occur via IP3-mediated mobilization of Ca2+ from intracellular stores and/or transmembrane influx of Ca2+ [ 22,  24].	transcription
71607	9	336202	7	NULL	NULL	NULL	NULL	IP3	Chemical		mediates					statement 8	Process				NULL		NULL	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_220	9915989	Nonetheless, although sphingosine-induced Ca2+ transients have been previously reported to occur via mobilization of Ca2+ from intracellular stores [ 33,  34], this study represents the first demonstration that ceramide regulates [Ca2+]i. Cch-induced Ca2+ transients occur via IP3-mediated mobilization of Ca2+ from intracellular stores and/or transmembrane influx of Ca2+ [ 22,  24].	transcription
71608	10	336202	7	NULL	NULL	0	NULL	statement 5	Process		occur via					statement 9	Process				NULL		0	NULL	NULL	NULL	gw60_biolreprod_60_2_262_s_220	9915989	Nonetheless, although sphingosine-induced Ca2+ transients have been previously reported to occur via mobilization of Ca2+ from intracellular stores [ 33,  34], this study represents the first demonstration that ceramide regulates [Ca2+]i. Cch-induced Ca2+ transients occur via IP3-mediated mobilization of Ca2+ from intracellular stores and/or transmembrane influx of Ca2+ [ 22,  24].	transcription
69575	1	336203	5	NULL	NULL	0	NULL	apoptosis	Process		is mediated by					Fas	GP				NULL	Jurkat T lymphocytes	0	NULL	NULL	NULL	gw60_molpharmacol_61_3_486_s_178	11854428	In contrast, sphingosine 1-phosphate (S1P), which protects Jurkat T lymphocytes from Fas- and ceramide-mediated apoptosis (Cuvillier et al., 1996  ), had a significant protective effect against FCCP-induced cell death; the percentage of apoptotic cells measured after 3 h of FCCP treatment decreasing from about 50 to 27% in the presence of 10 muM S1P.	transcription
69576	2	336203	5	NULL	NULL	0	NULL	apoptosis	Process		is mediated by					ceramide	Chemical				NULL	Jurkat T lymphocytes	0	NULL	NULL	NULL	gw60_molpharmacol_61_3_486_s_178	11854428	In contrast, sphingosine 1-phosphate (S1P), which protects Jurkat T lymphocytes from Fas- and ceramide-mediated apoptosis (Cuvillier et al., 1996  ), had a significant protective effect against FCCP-induced cell death; the percentage of apoptotic cells measured after 3 h of FCCP treatment decreasing from about 50 to 27% in the presence of 10 muM S1P.	transcription
69577	3	336203	5	NULL	NULL	0	NULL	S1P	Chemical		is					sphingosine 1-phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_3_486_s_178	11854428	In contrast, sphingosine 1-phosphate (S1P), which protects Jurkat T lymphocytes from Fas- and ceramide-mediated apoptosis (Cuvillier et al., 1996  ), had a significant protective effect against FCCP-induced cell death; the percentage of apoptotic cells measured after 3 h of FCCP treatment decreasing from about 50 to 27% in the presence of 10 muM S1P.	transcription
69578	4	336203	5	NULL	NULL	0	NULL	S1P	Chemical		protects					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_3_486_s_178	11854428	In contrast, sphingosine 1-phosphate (S1P), which protects Jurkat T lymphocytes from Fas- and ceramide-mediated apoptosis (Cuvillier et al., 1996  ), had a significant protective effect against FCCP-induced cell death; the percentage of apoptotic cells measured after 3 h of FCCP treatment decreasing from about 50 to 27% in the presence of 10 muM S1P.	transcription
69579	5	336203	5	NULL	NULL	0	NULL	S1P	Chemical		protects					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_3_486_s_178	11854428	In contrast, sphingosine 1-phosphate (S1P), which protects Jurkat T lymphocytes from Fas- and ceramide-mediated apoptosis (Cuvillier et al., 1996  ), had a significant protective effect against FCCP-induced cell death; the percentage of apoptotic cells measured after 3 h of FCCP treatment decreasing from about 50 to 27% in the presence of 10 muM S1P.	transcription
69580	6	336203	5	NULL	NULL	0	NULL	cell death	Process		is induced by					FCCP	Chemical				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_3_486_s_178	11854428	In contrast, sphingosine 1-phosphate (S1P), which protects Jurkat T lymphocytes from Fas- and ceramide-mediated apoptosis (Cuvillier et al., 1996  ), had a significant protective effect against FCCP-induced cell death; the percentage of apoptotic cells measured after 3 h of FCCP treatment decreasing from about 50 to 27% in the presence of 10 muM S1P.	transcription
69581	7	336203	5	NULL	NULL	0	NULL	S1P	Chemical		protects					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_3_486_s_178	11854428	In contrast, sphingosine 1-phosphate (S1P), which protects Jurkat T lymphocytes from Fas- and ceramide-mediated apoptosis (Cuvillier et al., 1996  ), had a significant protective effect against FCCP-induced cell death; the percentage of apoptotic cells measured after 3 h of FCCP treatment decreasing from about 50 to 27% in the presence of 10 muM S1P.	transcription
71609	1	336203	7	NULL	NULL	0	NULL	Fas	GP		mediates					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_3_486_s_178	11854428	In contrast, sphingosine 1-phosphate (S1P), which protects Jurkat T lymphocytes from Fas- and ceramide-mediated apoptosis (Cuvillier et al., 1996  ), had a significant protective effect against FCCP-induced cell death; the percentage of apoptotic cells measured after 3 h of FCCP treatment decreasing from about 50 to 27% in the presence of 10 muM S1P.	transcription
71610	2	336203	7	NULL	NULL	0	NULL	ceramide	Chemical		mediates					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_3_486_s_178	11854428	In contrast, sphingosine 1-phosphate (S1P), which protects Jurkat T lymphocytes from Fas- and ceramide-mediated apoptosis (Cuvillier et al., 1996  ), had a significant protective effect against FCCP-induced cell death; the percentage of apoptotic cells measured after 3 h of FCCP treatment decreasing from about 50 to 27% in the presence of 10 muM S1P.	transcription
71611	3	336203	7	NULL	NULL	0	NULL	S1P	Chemical		protects					Jurkat T lymphocytes	Cell				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_3_486_s_178	11854428	In contrast, sphingosine 1-phosphate (S1P), which protects Jurkat T lymphocytes from Fas- and ceramide-mediated apoptosis (Cuvillier et al., 1996  ), had a significant protective effect against FCCP-induced cell death; the percentage of apoptotic cells measured after 3 h of FCCP treatment decreasing from about 50 to 27% in the presence of 10 muM S1P.	transcription
71612	4	336203	7	NULL	NULL	0	NULL	Jurkat T lymphocytes	Cell		protected from					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_3_486_s_178	11854428	In contrast, sphingosine 1-phosphate (S1P), which protects Jurkat T lymphocytes from Fas- and ceramide-mediated apoptosis (Cuvillier et al., 1996  ), had a significant protective effect against FCCP-induced cell death; the percentage of apoptotic cells measured after 3 h of FCCP treatment decreasing from about 50 to 27% in the presence of 10 muM S1P.	transcription
71613	5	336203	7	NULL	NULL	0	NULL	Jurkat T lymphocytes	Cell		protected from					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_3_486_s_178	11854428	In contrast, sphingosine 1-phosphate (S1P), which protects Jurkat T lymphocytes from Fas- and ceramide-mediated apoptosis (Cuvillier et al., 1996  ), had a significant protective effect against FCCP-induced cell death; the percentage of apoptotic cells measured after 3 h of FCCP treatment decreasing from about 50 to 27% in the presence of 10 muM S1P.	transcription
71614	6	336203	7	NULL	NULL	0	NULL	FCCP	Chemical		induce					cell death	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_3_486_s_178	11854428	In contrast, sphingosine 1-phosphate (S1P), which protects Jurkat T lymphocytes from Fas- and ceramide-mediated apoptosis (Cuvillier et al., 1996  ), had a significant protective effect against FCCP-induced cell death; the percentage of apoptotic cells measured after 3 h of FCCP treatment decreasing from about 50 to 27% in the presence of 10 muM S1P.	transcription
71615	7	336203	7	NULL	NULL	0	NULL	S1P	Chemical		protect against		significantly			statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_3_486_s_178	11854428	In contrast, sphingosine 1-phosphate (S1P), which protects Jurkat T lymphocytes from Fas- and ceramide-mediated apoptosis (Cuvillier et al., 1996  ), had a significant protective effect against FCCP-induced cell death; the percentage of apoptotic cells measured after 3 h of FCCP treatment decreasing from about 50 to 27% in the presence of 10 muM S1P.	transcription
71616	8	336203	7	NULL	NULL	0	NULL	S1P	Chemical		is					sphingosine 1-phosphate	Chemical				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_61_3_486_s_178	11854428	In contrast, sphingosine 1-phosphate (S1P), which protects Jurkat T lymphocytes from Fas- and ceramide-mediated apoptosis (Cuvillier et al., 1996  ), had a significant protective effect against FCCP-induced cell death; the percentage of apoptotic cells measured after 3 h of FCCP treatment decreasing from about 50 to 27% in the presence of 10 muM S1P.	transcription
69582	1	336204	5	NULL	NULL	0	NULL	cell death	Process		is related to					sphingoid base	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_140	8626522	There was no evidence of apoptotic DNA damage  following exposure of HL-60 cells to fumonisin B   (100  muM) for 6 h; moreover, the extent of DNA fragmentation  elicited by exposure to sphingosine (10 muM) or sphinganine  (10 muM) for 6 h was not attenuated in the presence of  fumonisin B   ( Table 1 ), confirming that sphingoid  base-related cell death was not mediated by ceramide.	transcription
69583	2	336204	5	NULL	NULL	0	NULL	ceramide	Chemical		does not mediate					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_140	8626522	There was no evidence of apoptotic DNA damage  following exposure of HL-60 cells to fumonisin B   (100  muM) for 6 h; moreover, the extent of DNA fragmentation  elicited by exposure to sphingosine (10 muM) or sphinganine  (10 muM) for 6 h was not attenuated in the presence of  fumonisin B   ( Table 1 ), confirming that sphingoid  base-related cell death was not mediated by ceramide.	transcription
71617	1	336204	7	NULL	NULL	0	NULL	fumonisin B	Chemical		does not cause					apoptotic DNA damage	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_140	8626522	There was no evidence of apoptotic DNA damage  following exposure of HL-60 cells to fumonisin B   (100  muM) for 6 h; moreover, the extent of DNA fragmentation  elicited by exposure to sphingosine (10 muM) or sphinganine  (10 muM) for 6 h was not attenuated in the presence of  fumonisin B   ( Table 1 ), confirming that sphingoid  base-related cell death was not mediated by ceramide.	transcription
71618	2	336204	7	NULL	NULL	0	NULL	statement 1	Process		occur in					HL-60 cells 	Cell				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_140	8626522	There was no evidence of apoptotic DNA damage  following exposure of HL-60 cells to fumonisin B   (100  muM) for 6 h; moreover, the extent of DNA fragmentation  elicited by exposure to sphingosine (10 muM) or sphinganine  (10 muM) for 6 h was not attenuated in the presence of  fumonisin B   ( Table 1 ), confirming that sphingoid  base-related cell death was not mediated by ceramide.	transcription
71619	3	336204	7	NULL	NULL	0	NULL	sphingosine	Chemical		elicit					DNA fragmentation	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_140	8626522	There was no evidence of apoptotic DNA damage  following exposure of HL-60 cells to fumonisin B   (100  muM) for 6 h; moreover, the extent of DNA fragmentation  elicited by exposure to sphingosine (10 muM) or sphinganine  (10 muM) for 6 h was not attenuated in the presence of  fumonisin B   ( Table 1 ), confirming that sphingoid  base-related cell death was not mediated by ceramide.	transcription
71620	4	336204	7	NULL	NULL	0	NULL	sphinganine	Chemical		elicit					DNA fragmentation	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_140	8626522	There was no evidence of apoptotic DNA damage  following exposure of HL-60 cells to fumonisin B   (100  muM) for 6 h; moreover, the extent of DNA fragmentation  elicited by exposure to sphingosine (10 muM) or sphinganine  (10 muM) for 6 h was not attenuated in the presence of  fumonisin B   ( Table 1 ), confirming that sphingoid  base-related cell death was not mediated by ceramide.	transcription
71621	5	336204	7	NULL	NULL	0	NULL	fumonisin B 	Chemical		does not attenuate					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_140	8626522	There was no evidence of apoptotic DNA damage  following exposure of HL-60 cells to fumonisin B   (100  muM) for 6 h; moreover, the extent of DNA fragmentation  elicited by exposure to sphingosine (10 muM) or sphinganine  (10 muM) for 6 h was not attenuated in the presence of  fumonisin B   ( Table 1 ), confirming that sphingoid  base-related cell death was not mediated by ceramide.	transcription
71622	6	336204	7	NULL	NULL	0	NULL	fumonisin B  	Chemical		does not attenuate					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_140	8626522	There was no evidence of apoptotic DNA damage  following exposure of HL-60 cells to fumonisin B   (100  muM) for 6 h; moreover, the extent of DNA fragmentation  elicited by exposure to sphingosine (10 muM) or sphinganine  (10 muM) for 6 h was not attenuated in the presence of  fumonisin B   ( Table 1 ), confirming that sphingoid  base-related cell death was not mediated by ceramide.	transcription
71623	7	336204	7	NULL	NULL	0	NULL	sphingoid base	Chemical		relates to					cell death	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_140	8626522	There was no evidence of apoptotic DNA damage  following exposure of HL-60 cells to fumonisin B   (100  muM) for 6 h; moreover, the extent of DNA fragmentation  elicited by exposure to sphingosine (10 muM) or sphinganine  (10 muM) for 6 h was not attenuated in the presence of  fumonisin B   ( Table 1 ), confirming that sphingoid  base-related cell death was not mediated by ceramide.	transcription
71624	8	336204	7	NULL	NULL	0	NULL	ceramide	Chemical		does not mediate					statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_14_8275_s_140	8626522	There was no evidence of apoptotic DNA damage  following exposure of HL-60 cells to fumonisin B   (100  muM) for 6 h; moreover, the extent of DNA fragmentation  elicited by exposure to sphingosine (10 muM) or sphinganine  (10 muM) for 6 h was not attenuated in the presence of  fumonisin B   ( Table 1 ), confirming that sphingoid  base-related cell death was not mediated by ceramide.	transcription
69584	1	336205	5	NULL	NULL	0	NULL	trkA	GP	inhibition of	is required for		possibly			growth arrest	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_213	9278531	As similarly speculated by Posse de Chaves et al. (1997)  , when growth arrest and neurite retraction are required, it is anticipated that trkA functions would be inhibited, and engagement of p75NGFR would activate sphingomyelinase activity, leading to increased ceramide levels, and conversely, when survival and neurite extensions are required, trkA would not only suppress the ability of p75NGFR to stimulate sphingomyelinase, it would also stimulate sphingosine kinase and increase SPP levels.	transcription
69585	2	336205	5	NULL	NULL	0	NULL	trkA	GP	inhibition of	is required for		possibly			neurite	Cell	 retraction of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_213	9278531	As similarly speculated by Posse de Chaves et al. (1997)  , when growth arrest and neurite retraction are required, it is anticipated that trkA functions would be inhibited, and engagement of p75NGFR would activate sphingomyelinase activity, leading to increased ceramide levels, and conversely, when survival and neurite extensions are required, trkA would not only suppress the ability of p75NGFR to stimulate sphingomyelinase, it would also stimulate sphingosine kinase and increase SPP levels.	transcription
69586	3	336205	5	NULL	NULL	0	NULL	p75NGFR	GP	engagement of	activates		possibly			sphingomyelinase	GP				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_213	9278531	As similarly speculated by Posse de Chaves et al. (1997)  , when growth arrest and neurite retraction are required, it is anticipated that trkA functions would be inhibited, and engagement of p75NGFR would activate sphingomyelinase activity, leading to increased ceramide levels, and conversely, when survival and neurite extensions are required, trkA would not only suppress the ability of p75NGFR to stimulate sphingomyelinase, it would also stimulate sphingosine kinase and increase SPP levels.	transcription
69587	4	336205	5	NULL	NULL	0	NULL	statement 3	Process		leads to		possibly			ceramide	Chemical	increase in;;levels of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_213	9278531	As similarly speculated by Posse de Chaves et al. (1997)  , when growth arrest and neurite retraction are required, it is anticipated that trkA functions would be inhibited, and engagement of p75NGFR would activate sphingomyelinase activity, leading to increased ceramide levels, and conversely, when survival and neurite extensions are required, trkA would not only suppress the ability of p75NGFR to stimulate sphingomyelinase, it would also stimulate sphingosine kinase and increase SPP levels.	transcription
69588	5	336205	5	NULL	NULL	0	NULL	p75NGFR	GP		stimulates					sphingomyelinase	GP				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_213	9278531	As similarly speculated by Posse de Chaves et al. (1997)  , when growth arrest and neurite retraction are required, it is anticipated that trkA functions would be inhibited, and engagement of p75NGFR would activate sphingomyelinase activity, leading to increased ceramide levels, and conversely, when survival and neurite extensions are required, trkA would not only suppress the ability of p75NGFR to stimulate sphingomyelinase, it would also stimulate sphingosine kinase and increase SPP levels.	transcription
69589	6	336205	5	NULL	NULL	0	NULL	trkA	GP		suppress					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_213	9278531	As similarly speculated by Posse de Chaves et al. (1997)  , when growth arrest and neurite retraction are required, it is anticipated that trkA functions would be inhibited, and engagement of p75NGFR would activate sphingomyelinase activity, leading to increased ceramide levels, and conversely, when survival and neurite extensions are required, trkA would not only suppress the ability of p75NGFR to stimulate sphingomyelinase, it would also stimulate sphingosine kinase and increase SPP levels.	transcription
69591	7	336205	5	NULL	NULL	0	NULL	trkA	GP		stimulates					sphingosine kinase	GP				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_213	9278531	As similarly speculated by Posse de Chaves et al. (1997)  , when growth arrest and neurite retraction are required, it is anticipated that trkA functions would be inhibited, and engagement of p75NGFR would activate sphingomyelinase activity, leading to increased ceramide levels, and conversely, when survival and neurite extensions are required, trkA would not only suppress the ability of p75NGFR to stimulate sphingomyelinase, it would also stimulate sphingosine kinase and increase SPP levels.	transcription
69592	8	336205	5	NULL	NULL	0	NULL	statement 7	Process		increases					SPP	Chemical	level of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_213	9278531	As similarly speculated by Posse de Chaves et al. (1997)  , when growth arrest and neurite retraction are required, it is anticipated that trkA functions would be inhibited, and engagement of p75NGFR would activate sphingomyelinase activity, leading to increased ceramide levels, and conversely, when survival and neurite extensions are required, trkA would not only suppress the ability of p75NGFR to stimulate sphingomyelinase, it would also stimulate sphingosine kinase and increase SPP levels.	transcription
69593	9	336205	5	NULL	NULL	0	NULL	statement 6	Process		is required for		possibly			survival	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_213	9278531	As similarly speculated by Posse de Chaves et al. (1997)  , when growth arrest and neurite retraction are required, it is anticipated that trkA functions would be inhibited, and engagement of p75NGFR would activate sphingomyelinase activity, leading to increased ceramide levels, and conversely, when survival and neurite extensions are required, trkA would not only suppress the ability of p75NGFR to stimulate sphingomyelinase, it would also stimulate sphingosine kinase and increase SPP levels.	transcription
69594	10	336205	5	NULL	NULL	0	NULL	statement 6	Process		is required for		possibly			neurite	Cell	extension of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_213	9278531	As similarly speculated by Posse de Chaves et al. (1997)  , when growth arrest and neurite retraction are required, it is anticipated that trkA functions would be inhibited, and engagement of p75NGFR would activate sphingomyelinase activity, leading to increased ceramide levels, and conversely, when survival and neurite extensions are required, trkA would not only suppress the ability of p75NGFR to stimulate sphingomyelinase, it would also stimulate sphingosine kinase and increase SPP levels.	transcription
71625	1	336205	7	NULL	NULL	NULL	NULL	growth arrest	Process	requirement of	inhibit		may			trkA	GP	functions of			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_213	9278531	As similarly speculated by Posse de Chaves et al. (1997)  , when growth arrest and neurite retraction are required, it is anticipated that trkA functions would be inhibited, and engagement of p75NGFR would activate sphingomyelinase activity, leading to increased ceramide levels, and conversely, when survival and neurite extensions are required, trkA would not only suppress the ability of p75NGFR to stimulate sphingomyelinase, it would also stimulate sphingosine kinase and increase SPP levels.	transcription
71626	2	336205	7	NULL	NULL	NULL	NULL	 neurite retraction 	Process	requirement of	inhibit		may			 trkA	GP	functions of			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_213	9278531	As similarly speculated by Posse de Chaves et al. (1997)  , when growth arrest and neurite retraction are required, it is anticipated that trkA functions would be inhibited, and engagement of p75NGFR would activate sphingomyelinase activity, leading to increased ceramide levels, and conversely, when survival and neurite extensions are required, trkA would not only suppress the ability of p75NGFR to stimulate sphingomyelinase, it would also stimulate sphingosine kinase and increase SPP levels.	transcription
71627	3	336205	7	NULL	NULL	0	NULL	p75NGFR	GP		activate					sphingomyelinase	GP	activity of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_213	9278531	As similarly speculated by Posse de Chaves et al. (1997)  , when growth arrest and neurite retraction are required, it is anticipated that trkA functions would be inhibited, and engagement of p75NGFR would activate sphingomyelinase activity, leading to increased ceramide levels, and conversely, when survival and neurite extensions are required, trkA would not only suppress the ability of p75NGFR to stimulate sphingomyelinase, it would also stimulate sphingosine kinase and increase SPP levels.	transcription
71628	4	336205	7	NULL	NULL	0	NULL	statement 3	Process		leads to					ceramide levels	Chemical	increased			NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_213	9278531	As similarly speculated by Posse de Chaves et al. (1997)  , when growth arrest and neurite retraction are required, it is anticipated that trkA functions would be inhibited, and engagement of p75NGFR would activate sphingomyelinase activity, leading to increased ceramide levels, and conversely, when survival and neurite extensions are required, trkA would not only suppress the ability of p75NGFR to stimulate sphingomyelinase, it would also stimulate sphingosine kinase and increase SPP levels.	transcription
71629	5	336205	7	NULL	NULL	0	NULL	p75NGFR	GP		stimulate					sphingomyelinase	GP				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_213	9278531	As similarly speculated by Posse de Chaves et al. (1997)  , when growth arrest and neurite retraction are required, it is anticipated that trkA functions would be inhibited, and engagement of p75NGFR would activate sphingomyelinase activity, leading to increased ceramide levels, and conversely, when survival and neurite extensions are required, trkA would not only suppress the ability of p75NGFR to stimulate sphingomyelinase, it would also stimulate sphingosine kinase and increase SPP levels.	transcription
71630	6	336205	7	NULL	NULL	0	NULL	 trkA	GP		suppress					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_213	9278531	As similarly speculated by Posse de Chaves et al. (1997)  , when growth arrest and neurite retraction are required, it is anticipated that trkA functions would be inhibited, and engagement of p75NGFR would activate sphingomyelinase activity, leading to increased ceramide levels, and conversely, when survival and neurite extensions are required, trkA would not only suppress the ability of p75NGFR to stimulate sphingomyelinase, it would also stimulate sphingosine kinase and increase SPP levels.	transcription
71631	7	336205	7	NULL	NULL	0	NULL	trkA	GP		stimulate					sphingosine kinase	GP				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_213	9278531	As similarly speculated by Posse de Chaves et al. (1997)  , when growth arrest and neurite retraction are required, it is anticipated that trkA functions would be inhibited, and engagement of p75NGFR would activate sphingomyelinase activity, leading to increased ceramide levels, and conversely, when survival and neurite extensions are required, trkA would not only suppress the ability of p75NGFR to stimulate sphingomyelinase, it would also stimulate sphingosine kinase and increase SPP levels.	transcription
71632	8	336205	7	NULL	NULL	0	NULL	trkA	GP		increase					SPP	Chemical	levels of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_213	9278531	As similarly speculated by Posse de Chaves et al. (1997)  , when growth arrest and neurite retraction are required, it is anticipated that trkA functions would be inhibited, and engagement of p75NGFR would activate sphingomyelinase activity, leading to increased ceramide levels, and conversely, when survival and neurite extensions are required, trkA would not only suppress the ability of p75NGFR to stimulate sphingomyelinase, it would also stimulate sphingosine kinase and increase SPP levels.	transcription
71633	9	336205	7	NULL	NULL	0	NULL	statement 6	Process		occur upon					survival	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_213	9278531	As similarly speculated by Posse de Chaves et al. (1997)  , when growth arrest and neurite retraction are required, it is anticipated that trkA functions would be inhibited, and engagement of p75NGFR would activate sphingomyelinase activity, leading to increased ceramide levels, and conversely, when survival and neurite extensions are required, trkA would not only suppress the ability of p75NGFR to stimulate sphingomyelinase, it would also stimulate sphingosine kinase and increase SPP levels.	transcription
71634	10	336205	7	NULL	NULL	0	NULL	statement 6	Process		occur upon					neurite extenstions	Process	requirement of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_213	9278531	As similarly speculated by Posse de Chaves et al. (1997)  , when growth arrest and neurite retraction are required, it is anticipated that trkA functions would be inhibited, and engagement of p75NGFR would activate sphingomyelinase activity, leading to increased ceramide levels, and conversely, when survival and neurite extensions are required, trkA would not only suppress the ability of p75NGFR to stimulate sphingomyelinase, it would also stimulate sphingosine kinase and increase SPP levels.	transcription
71635	11	336205	7	NULL	NULL	0	NULL	statement 7	Process		occur upon					survival	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_213	9278531	As similarly speculated by Posse de Chaves et al. (1997)  , when growth arrest and neurite retraction are required, it is anticipated that trkA functions would be inhibited, and engagement of p75NGFR would activate sphingomyelinase activity, leading to increased ceramide levels, and conversely, when survival and neurite extensions are required, trkA would not only suppress the ability of p75NGFR to stimulate sphingomyelinase, it would also stimulate sphingosine kinase and increase SPP levels.	transcription
71636	12	336205	7	NULL	NULL	0	NULL	statement 7	Process		occur upon					neurite extenstions	Process	requirement of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_213	9278531	As similarly speculated by Posse de Chaves et al. (1997)  , when growth arrest and neurite retraction are required, it is anticipated that trkA functions would be inhibited, and engagement of p75NGFR would activate sphingomyelinase activity, leading to increased ceramide levels, and conversely, when survival and neurite extensions are required, trkA would not only suppress the ability of p75NGFR to stimulate sphingomyelinase, it would also stimulate sphingosine kinase and increase SPP levels.	transcription
71637	13	336205	7	NULL	NULL	0	NULL	statement 8	Process		occur upon					survival	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_213	9278531	As similarly speculated by Posse de Chaves et al. (1997)  , when growth arrest and neurite retraction are required, it is anticipated that trkA functions would be inhibited, and engagement of p75NGFR would activate sphingomyelinase activity, leading to increased ceramide levels, and conversely, when survival and neurite extensions are required, trkA would not only suppress the ability of p75NGFR to stimulate sphingomyelinase, it would also stimulate sphingosine kinase and increase SPP levels.	transcription
71638	14	336205	7	NULL	NULL	NULL	NULL	statement 8	Process		occur upon					neurite extenstions	Process	requirement of			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_17_18_6952_s_213	9278531	As similarly speculated by Posse de Chaves et al. (1997)  , when growth arrest and neurite retraction are required, it is anticipated that trkA functions would be inhibited, and engagement of p75NGFR would activate sphingomyelinase activity, leading to increased ceramide levels, and conversely, when survival and neurite extensions are required, trkA would not only suppress the ability of p75NGFR to stimulate sphingomyelinase, it would also stimulate sphingosine kinase and increase SPP levels.	transcription
69595	1	336206	5	NULL	NULL	0	NULL	FB1	Chemical		is					fumonisin B1	Chemical				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_22	9096129	We originally demonstrated that incubation with fumonisin B1 (FB1), a specific inhibitor of  N-acylation of the sphingoid long chain bases dihydrosphingosine (sphinganine) and sphingosine to dihydroceramide and ceramide, respectively (Merrill et al., 1996  ), disrupted axon growth during the early part of stage 3, between days 2 and 3 in culture (Harel and Futerman, 1993  ).	transcription
69596	2	336206	5	NULL	NULL	0	NULL	sphinganine	Chemical		is					dihydrosphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_22	9096129	We originally demonstrated that incubation with fumonisin B1 (FB1), a specific inhibitor of  N-acylation of the sphingoid long chain bases dihydrosphingosine (sphinganine) and sphingosine to dihydroceramide and ceramide, respectively (Merrill et al., 1996  ), disrupted axon growth during the early part of stage 3, between days 2 and 3 in culture (Harel and Futerman, 1993  ).	transcription
69597	3	336206	5	NULL	NULL	NULL	NULL	FB1	Chemical		is an inhibitor of		specific			dihydrosphingosine	Chemical	N-acylation of sphingoid long chain bases			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_22	9096129	We originally demonstrated that incubation with fumonisin B1 (FB1), a specific inhibitor of  N-acylation of the sphingoid long chain bases dihydrosphingosine (sphinganine) and sphingosine to dihydroceramide and ceramide, respectively (Merrill et al., 1996  ), disrupted axon growth during the early part of stage 3, between days 2 and 3 in culture (Harel and Futerman, 1993  ).	transcription
69598	4	336206	5	NULL	NULL	0	NULL	sphingosine	Chemical		is converted to					dihydroceramide 	Chemical				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_22	9096129	We originally demonstrated that incubation with fumonisin B1 (FB1), a specific inhibitor of  N-acylation of the sphingoid long chain bases dihydrosphingosine (sphinganine) and sphingosine to dihydroceramide and ceramide, respectively (Merrill et al., 1996  ), disrupted axon growth during the early part of stage 3, between days 2 and 3 in culture (Harel and Futerman, 1993  ).	transcription
69599	5	336206	5	NULL	NULL	0	NULL	sphingosine	Chemical		is converted to					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_22	9096129	We originally demonstrated that incubation with fumonisin B1 (FB1), a specific inhibitor of  N-acylation of the sphingoid long chain bases dihydrosphingosine (sphinganine) and sphingosine to dihydroceramide and ceramide, respectively (Merrill et al., 1996  ), disrupted axon growth during the early part of stage 3, between days 2 and 3 in culture (Harel and Futerman, 1993  ).	transcription
69600	6	336206	5	NULL	NULL	0	NULL	statement 4	Process		occurs along with					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_22	9096129	We originally demonstrated that incubation with fumonisin B1 (FB1), a specific inhibitor of  N-acylation of the sphingoid long chain bases dihydrosphingosine (sphinganine) and sphingosine to dihydroceramide and ceramide, respectively (Merrill et al., 1996  ), disrupted axon growth during the early part of stage 3, between days 2 and 3 in culture (Harel and Futerman, 1993  ).	transcription
69601	7	336206	5	NULL	NULL	0	NULL	FB1	Chemical		inhibits		specifically			statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_22	9096129	We originally demonstrated that incubation with fumonisin B1 (FB1), a specific inhibitor of  N-acylation of the sphingoid long chain bases dihydrosphingosine (sphinganine) and sphingosine to dihydroceramide and ceramide, respectively (Merrill et al., 1996  ), disrupted axon growth during the early part of stage 3, between days 2 and 3 in culture (Harel and Futerman, 1993  ).	transcription
69602	8	336206	5	NULL	NULL	0	NULL	FB1	Chemical		inhibits		specifically			statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_22	9096129	We originally demonstrated that incubation with fumonisin B1 (FB1), a specific inhibitor of  N-acylation of the sphingoid long chain bases dihydrosphingosine (sphinganine) and sphingosine to dihydroceramide and ceramide, respectively (Merrill et al., 1996  ), disrupted axon growth during the early part of stage 3, between days 2 and 3 in culture (Harel and Futerman, 1993  ).	transcription
69603	9	336206	5	NULL	NULL	NULL	NULL	FB1	Chemical		disrupts					axon	CellComponent	growth of			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_22	9096129	We originally demonstrated that incubation with fumonisin B1 (FB1), a specific inhibitor of  N-acylation of the sphingoid long chain bases dihydrosphingosine (sphinganine) and sphingosine to dihydroceramide and ceramide, respectively (Merrill et al., 1996  ), disrupted axon growth during the early part of stage 3, between days 2 and 3 in culture (Harel and Futerman, 1993  ).	transcription
71639	3	336206	7	NULL	NULL	NULL	NULL	FB1	Chemical		inhibit					statement 1	Process	 N-acylation of 			NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_22	9096129	We originally demonstrated that incubation with fumonisin B1 (FB1), a specific inhibitor of  N-acylation of the sphingoid long chain bases dihydrosphingosine (sphinganine) and sphingosine to dihydroceramide and ceramide, respectively (Merrill et al., 1996  ), disrupted axon growth during the early part of stage 3, between days 2 and 3 in culture (Harel and Futerman, 1993  ).	transcription
71640	1	336206	7	NULL	NULL	NULL	NULL	sphinganine	Chemical		acylated to					dihydroceramide	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_22	9096129	We originally demonstrated that incubation with fumonisin B1 (FB1), a specific inhibitor of  N-acylation of the sphingoid long chain bases dihydrosphingosine (sphinganine) and sphingosine to dihydroceramide and ceramide, respectively (Merrill et al., 1996  ), disrupted axon growth during the early part of stage 3, between days 2 and 3 in culture (Harel and Futerman, 1993  ).	transcription
71641	2	336206	7	NULL	NULL	NULL	NULL	 sphingosine 	Chemical		acylated to					ceramide	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_22	9096129	We originally demonstrated that incubation with fumonisin B1 (FB1), a specific inhibitor of  N-acylation of the sphingoid long chain bases dihydrosphingosine (sphinganine) and sphingosine to dihydroceramide and ceramide, respectively (Merrill et al., 1996  ), disrupted axon growth during the early part of stage 3, between days 2 and 3 in culture (Harel and Futerman, 1993  ).	transcription
71642	4	336206	7	NULL	NULL	0	NULL	FB1	Chemical		inhibit					statement 2	Process	N-acylation of			NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_22	9096129	We originally demonstrated that incubation with fumonisin B1 (FB1), a specific inhibitor of  N-acylation of the sphingoid long chain bases dihydrosphingosine (sphinganine) and sphingosine to dihydroceramide and ceramide, respectively (Merrill et al., 1996  ), disrupted axon growth during the early part of stage 3, between days 2 and 3 in culture (Harel and Futerman, 1993  ).	transcription
71643	5	336206	7	NULL	NULL	0	NULL	sphinganine	Chemical		is					dihydrosphingosine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_22	9096129	We originally demonstrated that incubation with fumonisin B1 (FB1), a specific inhibitor of  N-acylation of the sphingoid long chain bases dihydrosphingosine (sphinganine) and sphingosine to dihydroceramide and ceramide, respectively (Merrill et al., 1996  ), disrupted axon growth during the early part of stage 3, between days 2 and 3 in culture (Harel and Futerman, 1993  ).	transcription
71644	6	336206	7	NULL	NULL	0	NULL	dihydrosphingosine	Chemical		contains					sphingoid long chain bases	Chemical				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_22	9096129	We originally demonstrated that incubation with fumonisin B1 (FB1), a specific inhibitor of  N-acylation of the sphingoid long chain bases dihydrosphingosine (sphinganine) and sphingosine to dihydroceramide and ceramide, respectively (Merrill et al., 1996  ), disrupted axon growth during the early part of stage 3, between days 2 and 3 in culture (Harel and Futerman, 1993  ).	transcription
71645	7	336206	7	NULL	NULL	0	NULL	FB1	Chemical		disrupts					axon growth	Process				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_22	9096129	We originally demonstrated that incubation with fumonisin B1 (FB1), a specific inhibitor of  N-acylation of the sphingoid long chain bases dihydrosphingosine (sphinganine) and sphingosine to dihydroceramide and ceramide, respectively (Merrill et al., 1996  ), disrupted axon growth during the early part of stage 3, between days 2 and 3 in culture (Harel and Futerman, 1993  ).	transcription
71646	8	336206	7	NULL	NULL	0	NULL	FB1	Chemical		is					fumonisin B1	Chemical				NULL		0	NULL	NULL	NULL	gw60_jneurosci_17_9_2929_s_22	9096129	We originally demonstrated that incubation with fumonisin B1 (FB1), a specific inhibitor of  N-acylation of the sphingoid long chain bases dihydrosphingosine (sphinganine) and sphingosine to dihydroceramide and ceramide, respectively (Merrill et al., 1996  ), disrupted axon growth during the early part of stage 3, between days 2 and 3 in culture (Harel and Futerman, 1993  ).	transcription
69605	1	336209	5	NULL	NULL	0	NULL	capsiate	Chemical	sweet peppers	inhibits					NF-kappaB	GP	activation of			NULL	in vivo	0	NULL	NULL	NULL	gw60_neuropharmacology_44_7_958_s_328	12726827	Immunosuppressive activity of capsaicinoids: capsiate derived from sweet peppers inhibits NF-kappaB activation and is a potent antiinflammatory compound in vivo.	transcription
69606	2	336209	5	NULL	NULL	0	NULL	capsiate	Chemical		is a type of					capsaicinoids	Chemical				NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_44_7_958_s_328	12726827	Immunosuppressive activity of capsaicinoids: capsiate derived from sweet peppers inhibits NF-kappaB activation and is a potent antiinflammatory compound in vivo.	transcription
69607	3	336209	5	NULL	NULL	0	NULL	capsiate	Chemical		is a type of					potent antiinflammatory compound 	Chemical				NULL	in vivo	0	NULL	NULL	NULL	gw60_neuropharmacology_44_7_958_s_328	12726827	Immunosuppressive activity of capsaicinoids: capsiate derived from sweet peppers inhibits NF-kappaB activation and is a potent antiinflammatory compound in vivo.	transcription
71647	1	336209	7	NULL	NULL	0	NULL	capsiate	Chemical		derived from					sweet peppers	Organism				NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_44_7_958_s_328	12726827	Immunosuppressive activity of capsaicinoids: capsiate derived from sweet peppers inhibits NF-kappaB activation and is a potent antiinflammatory compound in vivo.	transcription
71648	2	336209	7	NULL	NULL	0	NULL	statement 1	Process		inhibits					NF-kappaB	GP	activation of			NULL	in vivo	0	NULL	NULL	NULL	gw60_neuropharmacology_44_7_958_s_328	12726827	Immunosuppressive activity of capsaicinoids: capsiate derived from sweet peppers inhibits NF-kappaB activation and is a potent antiinflammatory compound in vivo.	transcription
71649	3	336209	7	NULL	NULL	0	NULL	capsiate	Chemical		is a type of					potent antiinflammatory compound	Chemical				NULL	in vivo	0	NULL	NULL	NULL	gw60_neuropharmacology_44_7_958_s_328	12726827	Immunosuppressive activity of capsaicinoids: capsiate derived from sweet peppers inhibits NF-kappaB activation and is a potent antiinflammatory compound in vivo.	transcription
71650	4	336209	7	NULL	NULL	0	NULL	capsaicinoids	Chemical		shows					Immunosuppressive activity	Process				NULL		0	NULL	NULL	NULL	gw60_neuropharmacology_44_7_958_s_328	12726827	Immunosuppressive activity of capsaicinoids: capsiate derived from sweet peppers inhibits NF-kappaB activation and is a potent antiinflammatory compound in vivo.	transcription
69608	1	336212	5	NULL	NULL	NULL	NULL	HDL-apoE	GP		is involved in					lipoprotein	GP	metabolism of;;plasma			NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_44_5_884_s_22	12611904	It has been suggested that HDL-apoE is involved in several aspects of plasma lipoprotein metabolism, including  1) receptor-mediated delivery of HDL cholesterol to the liver ( ),  2) hepatic lipase-catalyzed hydrolysis of HDL phospholipid ( ),  3) plasma cholesterol esterification ( ),  4) plasma cholesteryl ester (CE) transfer ( ),  5) efflux of cell-derived cholesterol ( ,  ), and  6) stimulation of endothelial production of heparin sulfate ( ).	transcription
69609	2	336212	5	NULL	NULL	0	NULL	HDL cholesterol	Chemical		is delivered to					liver	OrganismPart				NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_5_884_s_22	12611904	It has been suggested that HDL-apoE is involved in several aspects of plasma lipoprotein metabolism, including  1) receptor-mediated delivery of HDL cholesterol to the liver ( ),  2) hepatic lipase-catalyzed hydrolysis of HDL phospholipid ( ),  3) plasma cholesterol esterification ( ),  4) plasma cholesteryl ester (CE) transfer ( ),  5) efflux of cell-derived cholesterol ( ,  ), and  6) stimulation of endothelial production of heparin sulfate ( ).	transcription
69610	3	336212	5	NULL	NULL	0	NULL	receptor	GP		mediates					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_5_884_s_22	12611904	It has been suggested that HDL-apoE is involved in several aspects of plasma lipoprotein metabolism, including  1) receptor-mediated delivery of HDL cholesterol to the liver ( ),  2) hepatic lipase-catalyzed hydrolysis of HDL phospholipid ( ),  3) plasma cholesterol esterification ( ),  4) plasma cholesteryl ester (CE) transfer ( ),  5) efflux of cell-derived cholesterol ( ,  ), and  6) stimulation of endothelial production of heparin sulfate ( ).	transcription
69611	4	336212	5	NULL	NULL	0	NULL	lipase	GP	hepatic	catalyzes					HDL phospholipid	Chemical	hydrolysis of 			NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_5_884_s_22	12611904	It has been suggested that HDL-apoE is involved in several aspects of plasma lipoprotein metabolism, including  1) receptor-mediated delivery of HDL cholesterol to the liver ( ),  2) hepatic lipase-catalyzed hydrolysis of HDL phospholipid ( ),  3) plasma cholesterol esterification ( ),  4) plasma cholesteryl ester (CE) transfer ( ),  5) efflux of cell-derived cholesterol ( ,  ), and  6) stimulation of endothelial production of heparin sulfate ( ).	transcription
69612	5	336212	5	NULL	NULL	NULL	NULL	statement 1	Process		includes					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_44_5_884_s_22	12611904	It has been suggested that HDL-apoE is involved in several aspects of plasma lipoprotein metabolism, including  1) receptor-mediated delivery of HDL cholesterol to the liver ( ),  2) hepatic lipase-catalyzed hydrolysis of HDL phospholipid ( ),  3) plasma cholesterol esterification ( ),  4) plasma cholesteryl ester (CE) transfer ( ),  5) efflux of cell-derived cholesterol ( ,  ), and  6) stimulation of endothelial production of heparin sulfate ( ).	transcription
69614	6	336212	5	NULL	NULL	0	NULL	statement 1	Process		includes					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_5_884_s_22	12611904	It has been suggested that HDL-apoE is involved in several aspects of plasma lipoprotein metabolism, including  1) receptor-mediated delivery of HDL cholesterol to the liver ( ),  2) hepatic lipase-catalyzed hydrolysis of HDL phospholipid ( ),  3) plasma cholesterol esterification ( ),  4) plasma cholesteryl ester (CE) transfer ( ),  5) efflux of cell-derived cholesterol ( ,  ), and  6) stimulation of endothelial production of heparin sulfate ( ).	transcription
69615	7	336212	5	NULL	NULL	NULL	NULL	HDL-apoE	GP		is involved in					cholesterol	Chemical	esterification of;;plasma 			NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_44_5_884_s_22	12611904	It has been suggested that HDL-apoE is involved in several aspects of plasma lipoprotein metabolism, including  1) receptor-mediated delivery of HDL cholesterol to the liver ( ),  2) hepatic lipase-catalyzed hydrolysis of HDL phospholipid ( ),  3) plasma cholesterol esterification ( ),  4) plasma cholesteryl ester (CE) transfer ( ),  5) efflux of cell-derived cholesterol ( ,  ), and  6) stimulation of endothelial production of heparin sulfate ( ).	transcription
69616	8	336212	5	NULL	NULL	0	NULL	HDL-apoE	GP		is involved in					cholesteryl ester	Chemical	transfer of;;plasma			NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_5_884_s_22	12611904	It has been suggested that HDL-apoE is involved in several aspects of plasma lipoprotein metabolism, including  1) receptor-mediated delivery of HDL cholesterol to the liver ( ),  2) hepatic lipase-catalyzed hydrolysis of HDL phospholipid ( ),  3) plasma cholesterol esterification ( ),  4) plasma cholesteryl ester (CE) transfer ( ),  5) efflux of cell-derived cholesterol ( ,  ), and  6) stimulation of endothelial production of heparin sulfate ( ).	transcription
69617	9	336212	5	NULL	NULL	0	NULL	HDL-apoE	GP		is involved in					cholesterol	Chemical	efflux of;;cell-derived			NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_5_884_s_22	12611904	It has been suggested that HDL-apoE is involved in several aspects of plasma lipoprotein metabolism, including  1) receptor-mediated delivery of HDL cholesterol to the liver ( ),  2) hepatic lipase-catalyzed hydrolysis of HDL phospholipid ( ),  3) plasma cholesterol esterification ( ),  4) plasma cholesteryl ester (CE) transfer ( ),  5) efflux of cell-derived cholesterol ( ,  ), and  6) stimulation of endothelial production of heparin sulfate ( ).	transcription
69618	10	336212	5	NULL	NULL	0	NULL	HDL-apoE	GP		is involved in					heparin sulfate	Chemical	stimulation of;;endothelial production of 			NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_5_884_s_22	12611904	It has been suggested that HDL-apoE is involved in several aspects of plasma lipoprotein metabolism, including  1) receptor-mediated delivery of HDL cholesterol to the liver ( ),  2) hepatic lipase-catalyzed hydrolysis of HDL phospholipid ( ),  3) plasma cholesterol esterification ( ),  4) plasma cholesteryl ester (CE) transfer ( ),  5) efflux of cell-derived cholesterol ( ,  ), and  6) stimulation of endothelial production of heparin sulfate ( ).	transcription
71651	1	336212	7	NULL	NULL	0	NULL	HDL-apoE	GP		is involved in					plasma lipoprotein metabolism	Process				NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_5_884_s_22	12611904	It has been suggested that HDL-apoE is involved in several aspects of plasma lipoprotein metabolism, including  1) receptor-mediated delivery of HDL cholesterol to the liver ( ),  2) hepatic lipase-catalyzed hydrolysis of HDL phospholipid ( ),  3) plasma cholesterol esterification ( ),  4) plasma cholesteryl ester (CE) transfer ( ),  5) efflux of cell-derived cholesterol ( ,  ), and  6) stimulation of endothelial production of heparin sulfate ( ).	transcription
71652	2	336212	7	NULL	NULL	0	NULL	HDL cholesterol	Chemical		delivered to					liver	OrganismPart				NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_5_884_s_22	12611904	It has been suggested that HDL-apoE is involved in several aspects of plasma lipoprotein metabolism, including  1) receptor-mediated delivery of HDL cholesterol to the liver ( ),  2) hepatic lipase-catalyzed hydrolysis of HDL phospholipid ( ),  3) plasma cholesterol esterification ( ),  4) plasma cholesteryl ester (CE) transfer ( ),  5) efflux of cell-derived cholesterol ( ,  ), and  6) stimulation of endothelial production of heparin sulfate ( ).	transcription
71653	3	336212	7	NULL	NULL	0	NULL	receptor	GP		mediates					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_5_884_s_22	12611904	It has been suggested that HDL-apoE is involved in several aspects of plasma lipoprotein metabolism, including  1) receptor-mediated delivery of HDL cholesterol to the liver ( ),  2) hepatic lipase-catalyzed hydrolysis of HDL phospholipid ( ),  3) plasma cholesterol esterification ( ),  4) plasma cholesteryl ester (CE) transfer ( ),  5) efflux of cell-derived cholesterol ( ,  ), and  6) stimulation of endothelial production of heparin sulfate ( ).	transcription
71654	4	336212	7	NULL	NULL	0	NULL	hepatic lipase	GP		catalyze					HDL phospholipid	Chemical	hydrolysis of			NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_5_884_s_22	12611904	It has been suggested that HDL-apoE is involved in several aspects of plasma lipoprotein metabolism, including  1) receptor-mediated delivery of HDL cholesterol to the liver ( ),  2) hepatic lipase-catalyzed hydrolysis of HDL phospholipid ( ),  3) plasma cholesterol esterification ( ),  4) plasma cholesteryl ester (CE) transfer ( ),  5) efflux of cell-derived cholesterol ( ,  ), and  6) stimulation of endothelial production of heparin sulfate ( ).	transcription
71655	5	336212	7	NULL	NULL	NULL	NULL	HDL-apoE	GP		is involved in					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_44_5_884_s_22	12611904	It has been suggested that HDL-apoE is involved in several aspects of plasma lipoprotein metabolism, including  1) receptor-mediated delivery of HDL cholesterol to the liver ( ),  2) hepatic lipase-catalyzed hydrolysis of HDL phospholipid ( ),  3) plasma cholesterol esterification ( ),  4) plasma cholesteryl ester (CE) transfer ( ),  5) efflux of cell-derived cholesterol ( ,  ), and  6) stimulation of endothelial production of heparin sulfate ( ).	transcription
71656	6	336212	7	NULL	NULL	NULL	NULL	HDL-apoE	GP		is involved in					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_jlipidres_44_5_884_s_22	12611904	It has been suggested that HDL-apoE is involved in several aspects of plasma lipoprotein metabolism, including  1) receptor-mediated delivery of HDL cholesterol to the liver ( ),  2) hepatic lipase-catalyzed hydrolysis of HDL phospholipid ( ),  3) plasma cholesterol esterification ( ),  4) plasma cholesteryl ester (CE) transfer ( ),  5) efflux of cell-derived cholesterol ( ,  ), and  6) stimulation of endothelial production of heparin sulfate ( ).	transcription
71657	7	336212	7	NULL	NULL	0	NULL	HDL-apoE	GP		is involved in					plasma cholesterol	Chemical	esterification of			NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_5_884_s_22	12611904	It has been suggested that HDL-apoE is involved in several aspects of plasma lipoprotein metabolism, including  1) receptor-mediated delivery of HDL cholesterol to the liver ( ),  2) hepatic lipase-catalyzed hydrolysis of HDL phospholipid ( ),  3) plasma cholesterol esterification ( ),  4) plasma cholesteryl ester (CE) transfer ( ),  5) efflux of cell-derived cholesterol ( ,  ), and  6) stimulation of endothelial production of heparin sulfate ( ).	transcription
71658	8	336212	7	NULL	NULL	0	NULL	HDL-apoE	GP		is involved in					plasma CE	Chemical	transfer of			NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_5_884_s_22	12611904	It has been suggested that HDL-apoE is involved in several aspects of plasma lipoprotein metabolism, including  1) receptor-mediated delivery of HDL cholesterol to the liver ( ),  2) hepatic lipase-catalyzed hydrolysis of HDL phospholipid ( ),  3) plasma cholesterol esterification ( ),  4) plasma cholesteryl ester (CE) transfer ( ),  5) efflux of cell-derived cholesterol ( ,  ), and  6) stimulation of endothelial production of heparin sulfate ( ).	transcription
71659	9	336212	7	NULL	NULL	0	NULL	cholesterol	Chemical		derived from					Cell	Cell				NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_5_884_s_22	12611904	It has been suggested that HDL-apoE is involved in several aspects of plasma lipoprotein metabolism, including  1) receptor-mediated delivery of HDL cholesterol to the liver ( ),  2) hepatic lipase-catalyzed hydrolysis of HDL phospholipid ( ),  3) plasma cholesterol esterification ( ),  4) plasma cholesteryl ester (CE) transfer ( ),  5) efflux of cell-derived cholesterol ( ,  ), and  6) stimulation of endothelial production of heparin sulfate ( ).	transcription
71660	10	336212	7	NULL	NULL	0	NULL	HDL-apoE	GP		is involved in					statement 9	Process				NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_5_884_s_22	12611904	It has been suggested that HDL-apoE is involved in several aspects of plasma lipoprotein metabolism, including  1) receptor-mediated delivery of HDL cholesterol to the liver ( ),  2) hepatic lipase-catalyzed hydrolysis of HDL phospholipid ( ),  3) plasma cholesterol esterification ( ),  4) plasma cholesteryl ester (CE) transfer ( ),  5) efflux of cell-derived cholesterol ( ,  ), and  6) stimulation of endothelial production of heparin sulfate ( ).	transcription
71661	11	336212	7	NULL	NULL	0	NULL	HDL-apoE	GP		is involved in					heparin sulfate	Chemical	stimulation of endothelial production of 			NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_5_884_s_22	12611904	It has been suggested that HDL-apoE is involved in several aspects of plasma lipoprotein metabolism, including  1) receptor-mediated delivery of HDL cholesterol to the liver ( ),  2) hepatic lipase-catalyzed hydrolysis of HDL phospholipid ( ),  3) plasma cholesterol esterification ( ),  4) plasma cholesteryl ester (CE) transfer ( ),  5) efflux of cell-derived cholesterol ( ,  ), and  6) stimulation of endothelial production of heparin sulfate ( ).	transcription
71662	12	336212	7	NULL	NULL	0	NULL	CE	Chemical		is					cholesteryl ester	Chemical				NULL		0	NULL	NULL	NULL	gw70_jlipidres_44_5_884_s_22	12611904	It has been suggested that HDL-apoE is involved in several aspects of plasma lipoprotein metabolism, including  1) receptor-mediated delivery of HDL cholesterol to the liver ( ),  2) hepatic lipase-catalyzed hydrolysis of HDL phospholipid ( ),  3) plasma cholesterol esterification ( ),  4) plasma cholesteryl ester (CE) transfer ( ),  5) efflux of cell-derived cholesterol ( ,  ), and  6) stimulation of endothelial production of heparin sulfate ( ).	transcription
71663	1	336213	7	NULL	NULL	0	NULL	smaller remnant particles	Chemical		diffuse into					arterial intima	OrganismPart				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2474_s_27	10521378	This is supported by experimental data showing the following: (1) smaller remnant particles can diffuse into the arterial intima, whereas large chylomicrons and VLDL (diameter >75 nm) are excluded from entering the vessel wall 13 ; (2) due to their reduced size, increased apoE content, and association with lipoprotein lipase, TRL remnants are more likely to be retained by heparan sulfate proteoglycans within the arterial intima 14 ;(3) TRL-induced cholesteryl ester accumulation by macrophages is dependent on the exposure of apoE epitopes through lipolysis of TRL 15 ; (4) lipoprotein lipase - mediated generation of TRL remnants results in the formation of lipolytic products, which are cytotoxic to macrophages 16  and which can increase endothelial cell layer permeability 17 ; and (5) increased activity of coagulation factor XII in patients with hypertriglyceridemia is dependent on TRL lipolysis.	transcription
71664	2	336213	7	NULL	NULL	0	NULL	TRL remnants	GP		retained within					arterial intima	OrganismPart				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2474_s_27	10521378	This is supported by experimental data showing the following: (1) smaller remnant particles can diffuse into the arterial intima, whereas large chylomicrons and VLDL (diameter >75 nm) are excluded from entering the vessel wall 13 ; (2) due to their reduced size, increased apoE content, and association with lipoprotein lipase, TRL remnants are more likely to be retained by heparan sulfate proteoglycans within the arterial intima 14 ;(3) TRL-induced cholesteryl ester accumulation by macrophages is dependent on the exposure of apoE epitopes through lipolysis of TRL 15 ; (4) lipoprotein lipase - mediated generation of TRL remnants results in the formation of lipolytic products, which are cytotoxic to macrophages 16  and which can increase endothelial cell layer permeability 17 ; and (5) increased activity of coagulation factor XII in patients with hypertriglyceridemia is dependent on TRL lipolysis.	transcription
71665	3	336213	7	NULL	NULL	0	NULL	TRL remnants	GP		retained by					heparan sulfate proteoglycans	Chemical				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2474_s_27	10521378	This is supported by experimental data showing the following: (1) smaller remnant particles can diffuse into the arterial intima, whereas large chylomicrons and VLDL (diameter >75 nm) are excluded from entering the vessel wall 13 ; (2) due to their reduced size, increased apoE content, and association with lipoprotein lipase, TRL remnants are more likely to be retained by heparan sulfate proteoglycans within the arterial intima 14 ;(3) TRL-induced cholesteryl ester accumulation by macrophages is dependent on the exposure of apoE epitopes through lipolysis of TRL 15 ; (4) lipoprotein lipase - mediated generation of TRL remnants results in the formation of lipolytic products, which are cytotoxic to macrophages 16  and which can increase endothelial cell layer permeability 17 ; and (5) increased activity of coagulation factor XII in patients with hypertriglyceridemia is dependent on TRL lipolysis.	transcription
71666	4	336213	7	NULL	NULL	0	NULL	TRL remnants	GP		are reduced in					size	Process				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2474_s_27	10521378	This is supported by experimental data showing the following: (1) smaller remnant particles can diffuse into the arterial intima, whereas large chylomicrons and VLDL (diameter >75 nm) are excluded from entering the vessel wall 13 ; (2) due to their reduced size, increased apoE content, and association with lipoprotein lipase, TRL remnants are more likely to be retained by heparan sulfate proteoglycans within the arterial intima 14 ;(3) TRL-induced cholesteryl ester accumulation by macrophages is dependent on the exposure of apoE epitopes through lipolysis of TRL 15 ; (4) lipoprotein lipase - mediated generation of TRL remnants results in the formation of lipolytic products, which are cytotoxic to macrophages 16  and which can increase endothelial cell layer permeability 17 ; and (5) increased activity of coagulation factor XII in patients with hypertriglyceridemia is dependent on TRL lipolysis.	transcription
71667	5	336213	7	NULL	NULL	0	NULL	statement 2	Process		due to					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2474_s_27	10521378	This is supported by experimental data showing the following: (1) smaller remnant particles can diffuse into the arterial intima, whereas large chylomicrons and VLDL (diameter >75 nm) are excluded from entering the vessel wall 13 ; (2) due to their reduced size, increased apoE content, and association with lipoprotein lipase, TRL remnants are more likely to be retained by heparan sulfate proteoglycans within the arterial intima 14 ;(3) TRL-induced cholesteryl ester accumulation by macrophages is dependent on the exposure of apoE epitopes through lipolysis of TRL 15 ; (4) lipoprotein lipase - mediated generation of TRL remnants results in the formation of lipolytic products, which are cytotoxic to macrophages 16  and which can increase endothelial cell layer permeability 17 ; and (5) increased activity of coagulation factor XII in patients with hypertriglyceridemia is dependent on TRL lipolysis.	transcription
71668	6	336213	7	NULL	NULL	0	NULL	TRL remnants	GP		contains					apoE content	GP	increased 			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2474_s_27	10521378	This is supported by experimental data showing the following: (1) smaller remnant particles can diffuse into the arterial intima, whereas large chylomicrons and VLDL (diameter >75 nm) are excluded from entering the vessel wall 13 ; (2) due to their reduced size, increased apoE content, and association with lipoprotein lipase, TRL remnants are more likely to be retained by heparan sulfate proteoglycans within the arterial intima 14 ;(3) TRL-induced cholesteryl ester accumulation by macrophages is dependent on the exposure of apoE epitopes through lipolysis of TRL 15 ; (4) lipoprotein lipase - mediated generation of TRL remnants results in the formation of lipolytic products, which are cytotoxic to macrophages 16  and which can increase endothelial cell layer permeability 17 ; and (5) increased activity of coagulation factor XII in patients with hypertriglyceridemia is dependent on TRL lipolysis.	transcription
71670	7	336213	7	NULL	NULL	0	NULL	statement 2	Process		due to					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2474_s_27	10521378	This is supported by experimental data showing the following: (1) smaller remnant particles can diffuse into the arterial intima, whereas large chylomicrons and VLDL (diameter >75 nm) are excluded from entering the vessel wall 13 ; (2) due to their reduced size, increased apoE content, and association with lipoprotein lipase, TRL remnants are more likely to be retained by heparan sulfate proteoglycans within the arterial intima 14 ;(3) TRL-induced cholesteryl ester accumulation by macrophages is dependent on the exposure of apoE epitopes through lipolysis of TRL 15 ; (4) lipoprotein lipase - mediated generation of TRL remnants results in the formation of lipolytic products, which are cytotoxic to macrophages 16  and which can increase endothelial cell layer permeability 17 ; and (5) increased activity of coagulation factor XII in patients with hypertriglyceridemia is dependent on TRL lipolysis.	transcription
71671	8	336213	7	NULL	NULL	0	NULL	TRL remnants	GP		associate with					lipoprotein lipase	GP				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2474_s_27	10521378	This is supported by experimental data showing the following: (1) smaller remnant particles can diffuse into the arterial intima, whereas large chylomicrons and VLDL (diameter >75 nm) are excluded from entering the vessel wall 13 ; (2) due to their reduced size, increased apoE content, and association with lipoprotein lipase, TRL remnants are more likely to be retained by heparan sulfate proteoglycans within the arterial intima 14 ;(3) TRL-induced cholesteryl ester accumulation by macrophages is dependent on the exposure of apoE epitopes through lipolysis of TRL 15 ; (4) lipoprotein lipase - mediated generation of TRL remnants results in the formation of lipolytic products, which are cytotoxic to macrophages 16  and which can increase endothelial cell layer permeability 17 ; and (5) increased activity of coagulation factor XII in patients with hypertriglyceridemia is dependent on TRL lipolysis.	transcription
71672	9	336213	7	NULL	NULL	0	NULL	statement 2	Process		due to					statement 8	Process				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2474_s_27	10521378	This is supported by experimental data showing the following: (1) smaller remnant particles can diffuse into the arterial intima, whereas large chylomicrons and VLDL (diameter >75 nm) are excluded from entering the vessel wall 13 ; (2) due to their reduced size, increased apoE content, and association with lipoprotein lipase, TRL remnants are more likely to be retained by heparan sulfate proteoglycans within the arterial intima 14 ;(3) TRL-induced cholesteryl ester accumulation by macrophages is dependent on the exposure of apoE epitopes through lipolysis of TRL 15 ; (4) lipoprotein lipase - mediated generation of TRL remnants results in the formation of lipolytic products, which are cytotoxic to macrophages 16  and which can increase endothelial cell layer permeability 17 ; and (5) increased activity of coagulation factor XII in patients with hypertriglyceridemia is dependent on TRL lipolysis.	transcription
71673	10	336213	7	NULL	NULL	0	NULL	TRL	GP		induce					 cholesteryl ester	Chemical	accumulation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2474_s_27	10521378	This is supported by experimental data showing the following: (1) smaller remnant particles can diffuse into the arterial intima, whereas large chylomicrons and VLDL (diameter >75 nm) are excluded from entering the vessel wall 13 ; (2) due to their reduced size, increased apoE content, and association with lipoprotein lipase, TRL remnants are more likely to be retained by heparan sulfate proteoglycans within the arterial intima 14 ;(3) TRL-induced cholesteryl ester accumulation by macrophages is dependent on the exposure of apoE epitopes through lipolysis of TRL 15 ; (4) lipoprotein lipase - mediated generation of TRL remnants results in the formation of lipolytic products, which are cytotoxic to macrophages 16  and which can increase endothelial cell layer permeability 17 ; and (5) increased activity of coagulation factor XII in patients with hypertriglyceridemia is dependent on TRL lipolysis.	transcription
71674	11	336213	7	NULL	NULL	0	NULL	statement 10	Process		occur by					macrophages	CellComponent				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2474_s_27	10521378	This is supported by experimental data showing the following: (1) smaller remnant particles can diffuse into the arterial intima, whereas large chylomicrons and VLDL (diameter >75 nm) are excluded from entering the vessel wall 13 ; (2) due to their reduced size, increased apoE content, and association with lipoprotein lipase, TRL remnants are more likely to be retained by heparan sulfate proteoglycans within the arterial intima 14 ;(3) TRL-induced cholesteryl ester accumulation by macrophages is dependent on the exposure of apoE epitopes through lipolysis of TRL 15 ; (4) lipoprotein lipase - mediated generation of TRL remnants results in the formation of lipolytic products, which are cytotoxic to macrophages 16  and which can increase endothelial cell layer permeability 17 ; and (5) increased activity of coagulation factor XII in patients with hypertriglyceridemia is dependent on TRL lipolysis.	transcription
71675	12	336213	7	NULL	NULL	0	NULL	statement 10	Process		is dependent on					apoE epitopes	GP	exposure of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2474_s_27	10521378	This is supported by experimental data showing the following: (1) smaller remnant particles can diffuse into the arterial intima, whereas large chylomicrons and VLDL (diameter >75 nm) are excluded from entering the vessel wall 13 ; (2) due to their reduced size, increased apoE content, and association with lipoprotein lipase, TRL remnants are more likely to be retained by heparan sulfate proteoglycans within the arterial intima 14 ;(3) TRL-induced cholesteryl ester accumulation by macrophages is dependent on the exposure of apoE epitopes through lipolysis of TRL 15 ; (4) lipoprotein lipase - mediated generation of TRL remnants results in the formation of lipolytic products, which are cytotoxic to macrophages 16  and which can increase endothelial cell layer permeability 17 ; and (5) increased activity of coagulation factor XII in patients with hypertriglyceridemia is dependent on TRL lipolysis.	transcription
71676	13	336213	7	NULL	NULL	0	NULL	statement 12	Process		occur through					TRL	GP	lipolysis of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2474_s_27	10521378	This is supported by experimental data showing the following: (1) smaller remnant particles can diffuse into the arterial intima, whereas large chylomicrons and VLDL (diameter >75 nm) are excluded from entering the vessel wall 13 ; (2) due to their reduced size, increased apoE content, and association with lipoprotein lipase, TRL remnants are more likely to be retained by heparan sulfate proteoglycans within the arterial intima 14 ;(3) TRL-induced cholesteryl ester accumulation by macrophages is dependent on the exposure of apoE epitopes through lipolysis of TRL 15 ; (4) lipoprotein lipase - mediated generation of TRL remnants results in the formation of lipolytic products, which are cytotoxic to macrophages 16  and which can increase endothelial cell layer permeability 17 ; and (5) increased activity of coagulation factor XII in patients with hypertriglyceridemia is dependent on TRL lipolysis.	transcription
71677	14	336213	7	NULL	NULL	0	NULL	lipoprotein lipase	GP		mediates					TRL remnants	GP	generation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2474_s_27	10521378	This is supported by experimental data showing the following: (1) smaller remnant particles can diffuse into the arterial intima, whereas large chylomicrons and VLDL (diameter >75 nm) are excluded from entering the vessel wall 13 ; (2) due to their reduced size, increased apoE content, and association with lipoprotein lipase, TRL remnants are more likely to be retained by heparan sulfate proteoglycans within the arterial intima 14 ;(3) TRL-induced cholesteryl ester accumulation by macrophages is dependent on the exposure of apoE epitopes through lipolysis of TRL 15 ; (4) lipoprotein lipase - mediated generation of TRL remnants results in the formation of lipolytic products, which are cytotoxic to macrophages 16  and which can increase endothelial cell layer permeability 17 ; and (5) increased activity of coagulation factor XII in patients with hypertriglyceridemia is dependent on TRL lipolysis.	transcription
71678	15	336213	7	NULL	NULL	0	NULL	statement 14	Process		results in					lipolytic products	Chemical	accumulation of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2474_s_27	10521378	This is supported by experimental data showing the following: (1) smaller remnant particles can diffuse into the arterial intima, whereas large chylomicrons and VLDL (diameter >75 nm) are excluded from entering the vessel wall 13 ; (2) due to their reduced size, increased apoE content, and association with lipoprotein lipase, TRL remnants are more likely to be retained by heparan sulfate proteoglycans within the arterial intima 14 ;(3) TRL-induced cholesteryl ester accumulation by macrophages is dependent on the exposure of apoE epitopes through lipolysis of TRL 15 ; (4) lipoprotein lipase - mediated generation of TRL remnants results in the formation of lipolytic products, which are cytotoxic to macrophages 16  and which can increase endothelial cell layer permeability 17 ; and (5) increased activity of coagulation factor XII in patients with hypertriglyceridemia is dependent on TRL lipolysis.	transcription
71679	16	336213	7	NULL	NULL	0	NULL	lipolytic products	Chemical		cytotoxic to					macrophages	CellComponent				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2474_s_27	10521378	This is supported by experimental data showing the following: (1) smaller remnant particles can diffuse into the arterial intima, whereas large chylomicrons and VLDL (diameter >75 nm) are excluded from entering the vessel wall 13 ; (2) due to their reduced size, increased apoE content, and association with lipoprotein lipase, TRL remnants are more likely to be retained by heparan sulfate proteoglycans within the arterial intima 14 ;(3) TRL-induced cholesteryl ester accumulation by macrophages is dependent on the exposure of apoE epitopes through lipolysis of TRL 15 ; (4) lipoprotein lipase - mediated generation of TRL remnants results in the formation of lipolytic products, which are cytotoxic to macrophages 16  and which can increase endothelial cell layer permeability 17 ; and (5) increased activity of coagulation factor XII in patients with hypertriglyceridemia is dependent on TRL lipolysis.	transcription
71680	17	336213	7	NULL	NULL	0	NULL	macrophages	CellComponent		increase					endothelial cell layer 	CellComponent	permeability of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2474_s_27	10521378	This is supported by experimental data showing the following: (1) smaller remnant particles can diffuse into the arterial intima, whereas large chylomicrons and VLDL (diameter >75 nm) are excluded from entering the vessel wall 13 ; (2) due to their reduced size, increased apoE content, and association with lipoprotein lipase, TRL remnants are more likely to be retained by heparan sulfate proteoglycans within the arterial intima 14 ;(3) TRL-induced cholesteryl ester accumulation by macrophages is dependent on the exposure of apoE epitopes through lipolysis of TRL 15 ; (4) lipoprotein lipase - mediated generation of TRL remnants results in the formation of lipolytic products, which are cytotoxic to macrophages 16  and which can increase endothelial cell layer permeability 17 ; and (5) increased activity of coagulation factor XII in patients with hypertriglyceridemia is dependent on TRL lipolysis.	transcription
71681	18	336213	7	NULL	NULL	0	NULL	coagulation factor XII	GP	increased activity of	is dependent on					TRL	GP	lipolysis of			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2474_s_27	10521378	This is supported by experimental data showing the following: (1) smaller remnant particles can diffuse into the arterial intima, whereas large chylomicrons and VLDL (diameter >75 nm) are excluded from entering the vessel wall 13 ; (2) due to their reduced size, increased apoE content, and association with lipoprotein lipase, TRL remnants are more likely to be retained by heparan sulfate proteoglycans within the arterial intima 14 ;(3) TRL-induced cholesteryl ester accumulation by macrophages is dependent on the exposure of apoE epitopes through lipolysis of TRL 15 ; (4) lipoprotein lipase - mediated generation of TRL remnants results in the formation of lipolytic products, which are cytotoxic to macrophages 16  and which can increase endothelial cell layer permeability 17 ; and (5) increased activity of coagulation factor XII in patients with hypertriglyceridemia is dependent on TRL lipolysis.	transcription
71682	19	336213	7	NULL	NULL	0	NULL	statement 18	Process		occur in					hypertriglyceridemia patients	Organism				NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2474_s_27	10521378	This is supported by experimental data showing the following: (1) smaller remnant particles can diffuse into the arterial intima, whereas large chylomicrons and VLDL (diameter >75 nm) are excluded from entering the vessel wall 13 ; (2) due to their reduced size, increased apoE content, and association with lipoprotein lipase, TRL remnants are more likely to be retained by heparan sulfate proteoglycans within the arterial intima 14 ;(3) TRL-induced cholesteryl ester accumulation by macrophages is dependent on the exposure of apoE epitopes through lipolysis of TRL 15 ; (4) lipoprotein lipase - mediated generation of TRL remnants results in the formation of lipolytic products, which are cytotoxic to macrophages 16  and which can increase endothelial cell layer permeability 17 ; and (5) increased activity of coagulation factor XII in patients with hypertriglyceridemia is dependent on TRL lipolysis.	transcription
71683	20	336213	7	NULL	NULL	0	NULL	 large chylomicrons 	Chemical		are excluded from					vessel wall	CellComponent	entering the			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2474_s_27	10521378	This is supported by experimental data showing the following: (1) smaller remnant particles can diffuse into the arterial intima, whereas large chylomicrons and VLDL (diameter >75 nm) are excluded from entering the vessel wall 13 ; (2) due to their reduced size, increased apoE content, and association with lipoprotein lipase, TRL remnants are more likely to be retained by heparan sulfate proteoglycans within the arterial intima 14 ;(3) TRL-induced cholesteryl ester accumulation by macrophages is dependent on the exposure of apoE epitopes through lipolysis of TRL 15 ; (4) lipoprotein lipase - mediated generation of TRL remnants results in the formation of lipolytic products, which are cytotoxic to macrophages 16  and which can increase endothelial cell layer permeability 17 ; and (5) increased activity of coagulation factor XII in patients with hypertriglyceridemia is dependent on TRL lipolysis.	transcription
71684	21	336213	7	NULL	NULL	0	NULL	VLDL	GP		are excluded from					vessel wall	CellComponent	entering the			NULL		0	NULL	NULL	NULL	gw60_arterthrombvascbiol_19_10_2474_s_27	10521378	This is supported by experimental data showing the following: (1) smaller remnant particles can diffuse into the arterial intima, whereas large chylomicrons and VLDL (diameter >75 nm) are excluded from entering the vessel wall 13 ; (2) due to their reduced size, increased apoE content, and association with lipoprotein lipase, TRL remnants are more likely to be retained by heparan sulfate proteoglycans within the arterial intima 14 ;(3) TRL-induced cholesteryl ester accumulation by macrophages is dependent on the exposure of apoE epitopes through lipolysis of TRL 15 ; (4) lipoprotein lipase - mediated generation of TRL remnants results in the formation of lipolytic products, which are cytotoxic to macrophages 16  and which can increase endothelial cell layer permeability 17 ; and (5) increased activity of coagulation factor XII in patients with hypertriglyceridemia is dependent on TRL lipolysis.	transcription
71685	1	336214	7	NULL	NULL	0	NULL	phosphatidylcholine	Chemical		synthesize					SM	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_24_14636_s_87	8662871	Previous studies have shown that SM is mainly synthesized by phosphatidylcholine:ceramide cholinephosphotransferase that catalyzes a base-exchange reaction between ceramide and phosphatidylcholine ( 18).	transcription
71686	2	336214	7	NULL	NULL	0	NULL	ceramide	Chemical		converted to					phosphatidylcholine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_24_14636_s_87	8662871	Previous studies have shown that SM is mainly synthesized by phosphatidylcholine:ceramide cholinephosphotransferase that catalyzes a base-exchange reaction between ceramide and phosphatidylcholine ( 18).	transcription
71687	3	336214	7	NULL	NULL	0	NULL	ceramide cholinephosphotransferase 	GP		catalyze					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_24_14636_s_87	8662871	Previous studies have shown that SM is mainly synthesized by phosphatidylcholine:ceramide cholinephosphotransferase that catalyzes a base-exchange reaction between ceramide and phosphatidylcholine ( 18).	transcription
71688	4	336214	7	NULL	NULL	0	NULL	statement 2	Process		is a type of					base-exchange reaction	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_271_24_14636_s_87	8662871	Previous studies have shown that SM is mainly synthesized by phosphatidylcholine:ceramide cholinephosphotransferase that catalyzes a base-exchange reaction between ceramide and phosphatidylcholine ( 18).	transcription
69620	1	336215	5	NULL	NULL	0	NULL	agonist	Chemical		induce					phosphatidylcholine	Chemical	hydrolysis of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_27_24090_s_35	11953426	Whereas the agonist-induced hydrolysis of phosphatidylcholine (PC) results in PA production, the cleavage of sphingomyelin (SM) leads to generation of ceramides.	transcription
69621	2	336215	5	NULL	NULL	0	NULL	statement 1	Process		results in					PA	Chemical	production of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_27_24090_s_35	11953426	Whereas the agonist-induced hydrolysis of phosphatidylcholine (PC) results in PA production, the cleavage of sphingomyelin (SM) leads to generation of ceramides.	transcription
69622	3	336215	5	NULL	NULL	0	NULL	sphingomyelin	Chemical	cleavage of	generates					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_27_24090_s_35	11953426	Whereas the agonist-induced hydrolysis of phosphatidylcholine (PC) results in PA production, the cleavage of sphingomyelin (SM) leads to generation of ceramides.	transcription
69623	4	336215	5	NULL	NULL	0	NULL	PC	Chemical		is					phosphatidylcholine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_27_24090_s_35	11953426	Whereas the agonist-induced hydrolysis of phosphatidylcholine (PC) results in PA production, the cleavage of sphingomyelin (SM) leads to generation of ceramides.	transcription
69624	5	336215	5	NULL	NULL	0	NULL	SM	Chemical		is					sphingomyelin	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_27_24090_s_35	11953426	Whereas the agonist-induced hydrolysis of phosphatidylcholine (PC) results in PA production, the cleavage of sphingomyelin (SM) leads to generation of ceramides.	transcription
71689	1	336215	7	NULL	NULL	0	NULL	agonist	Chemical		induce					PC	Chemical	hydrolysis of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_27_24090_s_35	11953426	Whereas the agonist-induced hydrolysis of phosphatidylcholine (PC) results in PA production, the cleavage of sphingomyelin (SM) leads to generation of ceramides.	transcription
71690	2	336215	7	NULL	NULL	0	NULL	PC	Chemical		is					phosphatidylcholine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_27_24090_s_35	11953426	Whereas the agonist-induced hydrolysis of phosphatidylcholine (PC) results in PA production, the cleavage of sphingomyelin (SM) leads to generation of ceramides.	transcription
71691	3	336215	7	NULL	NULL	0	NULL	statement 1	Process		results in					PA	Chemical	production of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_27_24090_s_35	11953426	Whereas the agonist-induced hydrolysis of phosphatidylcholine (PC) results in PA production, the cleavage of sphingomyelin (SM) leads to generation of ceramides.	transcription
71692	4	336215	7	NULL	NULL	0	NULL	SM	Chemical	cleavage of 	leads to					ceramide	Chemical	generation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_27_24090_s_35	11953426	Whereas the agonist-induced hydrolysis of phosphatidylcholine (PC) results in PA production, the cleavage of sphingomyelin (SM) leads to generation of ceramides.	transcription
71693	5	336215	7	NULL	NULL	0	NULL	SM	Chemical		is					sphingomyelin	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_27_24090_s_35	11953426	Whereas the agonist-induced hydrolysis of phosphatidylcholine (PC) results in PA production, the cleavage of sphingomyelin (SM) leads to generation of ceramides.	transcription
69625	1	336216	5	NULL	NULL	NULL	NULL	SM	Chemical	synthesis of	is mediated by					phosphatidylcholine:ceramide cholinephosphotransferase	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_1_33_s_16	14685263	SM synthesis is mediated by a phosphatidylcholine:ceramide cholinephosphotransferase,  or SM synthase, which transfers the phosphorylcholine moiety from phosphatidylcholine  (PC) onto the primary hydroxyl of ceramide, thus generating SM and diacylglycerol  (DAG;  ;  ;  ).	transcription
69637	2	336216	5	NULL	NULL	0	NULL	phosphorylcholine moiety	Chemical		is transfered from					phosphatidylcholine	Chemical				NULL		0	NULL	NULL	NULL	gw70_embo_23_1_33_s_16	14685263	SM synthesis is mediated by a phosphatidylcholine:ceramide cholinephosphotransferase,  or SM synthase, which transfers the phosphorylcholine moiety from phosphatidylcholine  (PC) onto the primary hydroxyl of ceramide, thus generating SM and diacylglycerol  (DAG;  ;  ;  ).	transcription
69638	3	336216	5	NULL	NULL	0	NULL	phosphorylcholine moiety	Chemical		is transfered onto					ceramide	Chemical	primary hydroxyl  of			NULL		0	NULL	NULL	NULL	gw70_embo_23_1_33_s_16	14685263	SM synthesis is mediated by a phosphatidylcholine:ceramide cholinephosphotransferase,  or SM synthase, which transfers the phosphorylcholine moiety from phosphatidylcholine  (PC) onto the primary hydroxyl of ceramide, thus generating SM and diacylglycerol  (DAG;  ;  ;  ).	transcription
69639	4	336216	5	NULL	NULL	0	NULL	statement 2	Process		occurs along with					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_embo_23_1_33_s_16	14685263	SM synthesis is mediated by a phosphatidylcholine:ceramide cholinephosphotransferase,  or SM synthase, which transfers the phosphorylcholine moiety from phosphatidylcholine  (PC) onto the primary hydroxyl of ceramide, thus generating SM and diacylglycerol  (DAG;  ;  ;  ).	transcription
69640	5	336216	5	NULL	NULL	NULL	NULL	phosphatidylcholine:ceramide cholinephosphotransferase	GP		is involved in					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_1_33_s_16	14685263	SM synthesis is mediated by a phosphatidylcholine:ceramide cholinephosphotransferase,  or SM synthase, which transfers the phosphorylcholine moiety from phosphatidylcholine  (PC) onto the primary hydroxyl of ceramide, thus generating SM and diacylglycerol  (DAG;  ;  ;  ).	transcription
69641	6	336216	5	NULL	NULL	NULL	NULL	phosphatidylcholine:ceramide cholinephosphotransferase	GP		is involved in					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_1_33_s_16	14685263	SM synthesis is mediated by a phosphatidylcholine:ceramide cholinephosphotransferase,  or SM synthase, which transfers the phosphorylcholine moiety from phosphatidylcholine  (PC) onto the primary hydroxyl of ceramide, thus generating SM and diacylglycerol  (DAG;  ;  ;  ).	transcription
69642	7	336216	5	NULL	NULL	NULL	NULL	SM synthase	GP		is a synonym of					phosphatidylcholine:ceramide cholinephosphotransferase	GP				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_1_33_s_16	14685263	SM synthesis is mediated by a phosphatidylcholine:ceramide cholinephosphotransferase,  or SM synthase, which transfers the phosphorylcholine moiety from phosphatidylcholine  (PC) onto the primary hydroxyl of ceramide, thus generating SM and diacylglycerol  (DAG;  ;  ;  ).	transcription
69644	9	336216	5	NULL	NULL	0	NULL	statement 4	Process		generates					SM	Chemical				NULL		0	NULL	NULL	NULL	gw70_embo_23_1_33_s_16	14685263	SM synthesis is mediated by a phosphatidylcholine:ceramide cholinephosphotransferase,  or SM synthase, which transfers the phosphorylcholine moiety from phosphatidylcholine  (PC) onto the primary hydroxyl of ceramide, thus generating SM and diacylglycerol  (DAG;  ;  ;  ).	transcription
69645	10	336216	5	NULL	NULL	0	NULL	statement 4	Process		generates					DAG	Chemical				NULL		0	NULL	NULL	NULL	gw70_embo_23_1_33_s_16	14685263	SM synthesis is mediated by a phosphatidylcholine:ceramide cholinephosphotransferase,  or SM synthase, which transfers the phosphorylcholine moiety from phosphatidylcholine  (PC) onto the primary hydroxyl of ceramide, thus generating SM and diacylglycerol  (DAG;  ;  ;  ).	transcription
69646	11	336216	5	NULL	NULL	0	NULL	DAG	Chemical		is					diacylglycerol	Chemical				NULL		0	NULL	NULL	NULL	gw70_embo_23_1_33_s_16	14685263	SM synthesis is mediated by a phosphatidylcholine:ceramide cholinephosphotransferase,  or SM synthase, which transfers the phosphorylcholine moiety from phosphatidylcholine  (PC) onto the primary hydroxyl of ceramide, thus generating SM and diacylglycerol  (DAG;  ;  ;  ).	transcription
69647	8	336216	5	NULL	NULL	NULL	NULL	PC	Chemical		is					phosphatidylcholine	Chemical				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_1_33_s_16	14685263	SM synthesis is mediated by a phosphatidylcholine:ceramide cholinephosphotransferase,  or SM synthase, which transfers the phosphorylcholine moiety from phosphatidylcholine  (PC) onto the primary hydroxyl of ceramide, thus generating SM and diacylglycerol  (DAG;  ;  ;  ).	transcription
71694	1	336216	7	NULL	NULL	0	NULL	SM	Chemical	synthesis of	mediated by					phosphatidylcholine	Chemical				NULL		0	NULL	NULL	NULL	gw70_embo_23_1_33_s_16	14685263	SM synthesis is mediated by a phosphatidylcholine:ceramide cholinephosphotransferase,  or SM synthase, which transfers the phosphorylcholine moiety from phosphatidylcholine  (PC) onto the primary hydroxyl of ceramide, thus generating SM and diacylglycerol  (DAG;  ;  ;  ).	transcription
71695	2	336216	7	NULL	NULL	NULL	NULL	PC	Chemical	phosphorylcholine moiety of	transferred to					ceramide	Chemical	primary hydroxyl of			NULL		NULL	NULL	NULL	NULL	gw70_embo_23_1_33_s_16	14685263	SM synthesis is mediated by a phosphatidylcholine:ceramide cholinephosphotransferase,  or SM synthase, which transfers the phosphorylcholine moiety from phosphatidylcholine  (PC) onto the primary hydroxyl of ceramide, thus generating SM and diacylglycerol  (DAG;  ;  ;  ).	transcription
71696	3	336216	7	NULL	NULL	NULL	NULL	ceramide cholinephosphotransferase	Chemical		catalyze					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_embo_23_1_33_s_16	14685263	SM synthesis is mediated by a phosphatidylcholine:ceramide cholinephosphotransferase,  or SM synthase, which transfers the phosphorylcholine moiety from phosphatidylcholine  (PC) onto the primary hydroxyl of ceramide, thus generating SM and diacylglycerol  (DAG;  ;  ;  ).	transcription
71697	4	336216	7	NULL	NULL	0	NULL	SM synthase	GP		catalyze					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_embo_23_1_33_s_16	14685263	SM synthesis is mediated by a phosphatidylcholine:ceramide cholinephosphotransferase,  or SM synthase, which transfers the phosphorylcholine moiety from phosphatidylcholine  (PC) onto the primary hydroxyl of ceramide, thus generating SM and diacylglycerol  (DAG;  ;  ;  ).	transcription
71698	5	336216	7	NULL	NULL	0	NULL	statement 2	Process		generate					SM	Chemical				NULL		0	NULL	NULL	NULL	gw70_embo_23_1_33_s_16	14685263	SM synthesis is mediated by a phosphatidylcholine:ceramide cholinephosphotransferase,  or SM synthase, which transfers the phosphorylcholine moiety from phosphatidylcholine  (PC) onto the primary hydroxyl of ceramide, thus generating SM and diacylglycerol  (DAG;  ;  ;  ).	transcription
71699	6	336216	7	NULL	NULL	0	NULL	statement 2	Process		generate					DAG					NULL		0	NULL	NULL	NULL	gw70_embo_23_1_33_s_16	14685263	SM synthesis is mediated by a phosphatidylcholine:ceramide cholinephosphotransferase,  or SM synthase, which transfers the phosphorylcholine moiety from phosphatidylcholine  (PC) onto the primary hydroxyl of ceramide, thus generating SM and diacylglycerol  (DAG;  ;  ;  ).	transcription
71700	7	336216	7	NULL	NULL	0	NULL	statement 5	Process		occur along with					statement 6	Process				NULL		0	NULL	NULL	NULL	gw70_embo_23_1_33_s_16	14685263	SM synthesis is mediated by a phosphatidylcholine:ceramide cholinephosphotransferase,  or SM synthase, which transfers the phosphorylcholine moiety from phosphatidylcholine  (PC) onto the primary hydroxyl of ceramide, thus generating SM and diacylglycerol  (DAG;  ;  ;  ).	transcription
71701	8	336216	7	NULL	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_embo_23_1_33_s_16	14685263	SM synthesis is mediated by a phosphatidylcholine:ceramide cholinephosphotransferase,  or SM synthase, which transfers the phosphorylcholine moiety from phosphatidylcholine  (PC) onto the primary hydroxyl of ceramide, thus generating SM and diacylglycerol  (DAG;  ;  ;  ).	transcription
71702	9	336216	7	NULL	NULL	0	NULL	PC	Chemical		is					phosphatidylcholine	Chemical				NULL		0	NULL	NULL	NULL	gw70_embo_23_1_33_s_16	14685263	SM synthesis is mediated by a phosphatidylcholine:ceramide cholinephosphotransferase,  or SM synthase, which transfers the phosphorylcholine moiety from phosphatidylcholine  (PC) onto the primary hydroxyl of ceramide, thus generating SM and diacylglycerol  (DAG;  ;  ;  ).	transcription
71703	10	336216	7	NULL	NULL	0	NULL	DAG	Chemical		is					diacylglycerol	Chemical				NULL		0	NULL	NULL	NULL	gw70_embo_23_1_33_s_16	14685263	SM synthesis is mediated by a phosphatidylcholine:ceramide cholinephosphotransferase,  or SM synthase, which transfers the phosphorylcholine moiety from phosphatidylcholine  (PC) onto the primary hydroxyl of ceramide, thus generating SM and diacylglycerol  (DAG;  ;  ;  ).	transcription
69648	1	336217	5	NULL	NULL	0	NULL	Bid	GP		is translocated to					mitochondria	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_12_10073_s_370	11790791	Translocation of Bid to the Mitochondria with Ceramide--  Upon activation the Fas receptor generated ceramide, as a consequence of the sequential involvement of phosphatidylcholine-specific phospholipase C and an acidic sphingomyelinase ( 42).	transcription
69649	2	336217	5	NULL	NULL	0	NULL	statement 1	Process		occurs along with					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_12_10073_s_370	11790791	Translocation of Bid to the Mitochondria with Ceramide--  Upon activation the Fas receptor generated ceramide, as a consequence of the sequential involvement of phosphatidylcholine-specific phospholipase C and an acidic sphingomyelinase ( 42).	transcription
69650	3	336217	5	NULL	NULL	NULL	NULL	ceramide	Chemical		is generated by					Fas receptor	GP	activated			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10073_s_370	11790791	Translocation of Bid to the Mitochondria with Ceramide--  Upon activation the Fas receptor generated ceramide, as a consequence of the sequential involvement of phosphatidylcholine-specific phospholipase C and an acidic sphingomyelinase ( 42).	transcription
69651	4	336217	5	NULL	NULL	0	NULL	phospholipase C	GP		is specific to					phosphatidylcholine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_12_10073_s_370	11790791	Translocation of Bid to the Mitochondria with Ceramide--  Upon activation the Fas receptor generated ceramide, as a consequence of the sequential involvement of phosphatidylcholine-specific phospholipase C and an acidic sphingomyelinase ( 42).	transcription
69653	5	336217	5	NULL	NULL	0	NULL	statement 4	GP		is involved in		sequential			statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_12_10073_s_370	11790791	Translocation of Bid to the Mitochondria with Ceramide--  Upon activation the Fas receptor generated ceramide, as a consequence of the sequential involvement of phosphatidylcholine-specific phospholipase C and an acidic sphingomyelinase ( 42).	transcription
69654	6	336217	5	NULL	NULL	0	NULL	sphingomyelinase	GP	acidic	is involved in		sequential			statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_12_10073_s_370	11790791	Translocation of Bid to the Mitochondria with Ceramide--  Upon activation the Fas receptor generated ceramide, as a consequence of the sequential involvement of phosphatidylcholine-specific phospholipase C and an acidic sphingomyelinase ( 42).	transcription
71704	1	336217	7	NULL	NULL	0	NULL	Bid	GP		translocated to					mitochondria	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_12_10073_s_370	11790791	Translocation of Bid to the Mitochondria with Ceramide--  Upon activation the Fas receptor generated ceramide, as a consequence of the sequential involvement of phosphatidylcholine-specific phospholipase C and an acidic sphingomyelinase ( 42).	transcription
71705	2	336217	7	NULL	NULL	0	NULL	ceramide	Chemical		translocated to					mitochondria	CellComponent				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_12_10073_s_370	11790791	Translocation of Bid to the Mitochondria with Ceramide--  Upon activation the Fas receptor generated ceramide, as a consequence of the sequential involvement of phosphatidylcholine-specific phospholipase C and an acidic sphingomyelinase ( 42).	transcription
71706	3	336217	7	NULL	NULL	0	NULL	statement 1	Process		occur along with					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_12_10073_s_370	11790791	Translocation of Bid to the Mitochondria with Ceramide--  Upon activation the Fas receptor generated ceramide, as a consequence of the sequential involvement of phosphatidylcholine-specific phospholipase C and an acidic sphingomyelinase ( 42).	transcription
71707	4	336217	7	NULL	NULL	0	NULL	 Fas receptor	GP	activation of	generates					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_12_10073_s_370	11790791	Translocation of Bid to the Mitochondria with Ceramide--  Upon activation the Fas receptor generated ceramide, as a consequence of the sequential involvement of phosphatidylcholine-specific phospholipase C and an acidic sphingomyelinase ( 42).	transcription
71708	5	336217	7	NULL	NULL	NULL	NULL	statement 4	Process		involves					phosphatidylcholine-specific phospholipase C	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10073_s_370	11790791	Translocation of Bid to the Mitochondria with Ceramide--  Upon activation the Fas receptor generated ceramide, as a consequence of the sequential involvement of phosphatidylcholine-specific phospholipase C and an acidic sphingomyelinase ( 42).	transcription
71709	6	336217	7	NULL	NULL	NULL	NULL	statement 4	Process		involves					acidic sphingomyelinase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_277_12_10073_s_370	11790791	Translocation of Bid to the Mitochondria with Ceramide--  Upon activation the Fas receptor generated ceramide, as a consequence of the sequential involvement of phosphatidylcholine-specific phospholipase C and an acidic sphingomyelinase ( 42).	transcription
71710	7	336217	7	NULL	NULL	0	NULL	statement 6	Process		occur after					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_12_10073_s_370	11790791	Translocation of Bid to the Mitochondria with Ceramide--  Upon activation the Fas receptor generated ceramide, as a consequence of the sequential involvement of phosphatidylcholine-specific phospholipase C and an acidic sphingomyelinase ( 42).	transcription
69655	1	336218	5	NULL	NULL	0	NULL	phosphatidylcholine:ceramide phosphocholine transferase	GP		regulates					ceramide	Chemical	level of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_23_14550_s_35	9603970	One of the most intriguing enzymes that regulate ceramide levels is the phosphatidylcholine:ceramide phosphocholine transferase (sphingomyelin synthase; SMS), which transfers the phosphocholine group from PC to ceramide generating sphingomyelin (SM) and DAG ( 27-33).	transcription
69656	2	336218	5	NULL	NULL	0	NULL	phosphatidylcholine:ceramide phosphocholine transferase	GP		is a synonym of					sphingomyelin synthase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_23_14550_s_35	9603970	One of the most intriguing enzymes that regulate ceramide levels is the phosphatidylcholine:ceramide phosphocholine transferase (sphingomyelin synthase; SMS), which transfers the phosphocholine group from PC to ceramide generating sphingomyelin (SM) and DAG ( 27-33).	transcription
69657	3	336218	5	NULL	NULL	0	NULL	sphingomyelin synthase	GP		is					SMS	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_23_14550_s_35	9603970	One of the most intriguing enzymes that regulate ceramide levels is the phosphatidylcholine:ceramide phosphocholine transferase (sphingomyelin synthase; SMS), which transfers the phosphocholine group from PC to ceramide generating sphingomyelin (SM) and DAG ( 27-33).	transcription
69658	4	336218	5	NULL	NULL	NULL	NULL	phosphocholine group	Chemical		is transfered from					PC	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_23_14550_s_35	9603970	One of the most intriguing enzymes that regulate ceramide levels is the phosphatidylcholine:ceramide phosphocholine transferase (sphingomyelin synthase; SMS), which transfers the phosphocholine group from PC to ceramide generating sphingomyelin (SM) and DAG ( 27-33).	transcription
69659	5	336218	5	NULL	NULL	0	NULL	phosphocholine group	Chemical		is transfered to					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_23_14550_s_35	9603970	One of the most intriguing enzymes that regulate ceramide levels is the phosphatidylcholine:ceramide phosphocholine transferase (sphingomyelin synthase; SMS), which transfers the phosphocholine group from PC to ceramide generating sphingomyelin (SM) and DAG ( 27-33).	transcription
69660	6	336218	5	NULL	NULL	0	NULL	statement 4	Process		occurs along with					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_23_14550_s_35	9603970	One of the most intriguing enzymes that regulate ceramide levels is the phosphatidylcholine:ceramide phosphocholine transferase (sphingomyelin synthase; SMS), which transfers the phosphocholine group from PC to ceramide generating sphingomyelin (SM) and DAG ( 27-33).	transcription
69661	7	336218	5	NULL	NULL	0	NULL	statement 6	Process		generates					SM	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_23_14550_s_35	9603970	One of the most intriguing enzymes that regulate ceramide levels is the phosphatidylcholine:ceramide phosphocholine transferase (sphingomyelin synthase; SMS), which transfers the phosphocholine group from PC to ceramide generating sphingomyelin (SM) and DAG ( 27-33).	transcription
69662	8	336218	5	NULL	NULL	0	NULL	statement 6	Process		generates					DAG	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_23_14550_s_35	9603970	One of the most intriguing enzymes that regulate ceramide levels is the phosphatidylcholine:ceramide phosphocholine transferase (sphingomyelin synthase; SMS), which transfers the phosphocholine group from PC to ceramide generating sphingomyelin (SM) and DAG ( 27-33).	transcription
69663	9	336218	5	NULL	NULL	0	NULL	SM	Chemical		is					sphingomyelin	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_23_14550_s_35	9603970	One of the most intriguing enzymes that regulate ceramide levels is the phosphatidylcholine:ceramide phosphocholine transferase (sphingomyelin synthase; SMS), which transfers the phosphocholine group from PC to ceramide generating sphingomyelin (SM) and DAG ( 27-33).	transcription
71711	1	336218	7	NULL	NULL	0	NULL	 PC	Chemical	phosphocholine group from	transferred to					 ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_23_14550_s_35	9603970	One of the most intriguing enzymes that regulate ceramide levels is the phosphatidylcholine:ceramide phosphocholine transferase (sphingomyelin synthase; SMS), which transfers the phosphocholine group from PC to ceramide generating sphingomyelin (SM) and DAG ( 27-33).	transcription
71712	2	336218	7	NULL	NULL	0	NULL	phosphatidylcholine:ceramide phosphocholine transferase	GP		catalyze					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_23_14550_s_35	9603970	One of the most intriguing enzymes that regulate ceramide levels is the phosphatidylcholine:ceramide phosphocholine transferase (sphingomyelin synthase; SMS), which transfers the phosphocholine group from PC to ceramide generating sphingomyelin (SM) and DAG ( 27-33).	transcription
71713	3	336218	7	NULL	NULL	0	NULL	statement 1	Process		generate					SM	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_23_14550_s_35	9603970	One of the most intriguing enzymes that regulate ceramide levels is the phosphatidylcholine:ceramide phosphocholine transferase (sphingomyelin synthase; SMS), which transfers the phosphocholine group from PC to ceramide generating sphingomyelin (SM) and DAG ( 27-33).	transcription
71714	4	336218	7	NULL	NULL	0	NULL	statement 1	Process		generate					DAG	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_23_14550_s_35	9603970	One of the most intriguing enzymes that regulate ceramide levels is the phosphatidylcholine:ceramide phosphocholine transferase (sphingomyelin synthase; SMS), which transfers the phosphocholine group from PC to ceramide generating sphingomyelin (SM) and DAG ( 27-33).	transcription
71715	5	336218	7	NULL	NULL	0	NULL	SM	Chemical		is					sphingomyelin 	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_23_14550_s_35	9603970	One of the most intriguing enzymes that regulate ceramide levels is the phosphatidylcholine:ceramide phosphocholine transferase (sphingomyelin synthase; SMS), which transfers the phosphocholine group from PC to ceramide generating sphingomyelin (SM) and DAG ( 27-33).	transcription
71716	6	336218	7	NULL	NULL	0	NULL	phosphatidylcholine:ceramide phosphocholine transferase	GP		is					SMS	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_23_14550_s_35	9603970	One of the most intriguing enzymes that regulate ceramide levels is the phosphatidylcholine:ceramide phosphocholine transferase (sphingomyelin synthase; SMS), which transfers the phosphocholine group from PC to ceramide generating sphingomyelin (SM) and DAG ( 27-33).	transcription
71717	7	336218	7	NULL	NULL	0	NULL	SMS	GP		is					sphingomyelin synthase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_23_14550_s_35	9603970	One of the most intriguing enzymes that regulate ceramide levels is the phosphatidylcholine:ceramide phosphocholine transferase (sphingomyelin synthase; SMS), which transfers the phosphocholine group from PC to ceramide generating sphingomyelin (SM) and DAG ( 27-33).	transcription
71719	8	336218	7	NULL	NULL	NULL	NULL	SMS	GP		regulate					ceramide	Chemical	levels of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_23_14550_s_35	9603970	One of the most intriguing enzymes that regulate ceramide levels is the phosphatidylcholine:ceramide phosphocholine transferase (sphingomyelin synthase; SMS), which transfers the phosphocholine group from PC to ceramide generating sphingomyelin (SM) and DAG ( 27-33).	transcription
69665	1	336219	5	NULL	NULL	0	NULL	ceramide	Chemical		induce		potentially			programmed cell death	Process				NULL	lung cells	0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_15	15772421	Ceramide potently induces programmed cell death in lung cells and inhibits the biosynthesis of phosphatidylcholine (PtdCho), the predominant phospholipid of alveolar surfactant ( ,   -  ).	transcription
69666	2	336219	5	NULL	NULL	0	NULL	ceramide	Chemical		inhibits					PtdCho	Chemical	biosynthesis of			NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_15	15772421	Ceramide potently induces programmed cell death in lung cells and inhibits the biosynthesis of phosphatidylcholine (PtdCho), the predominant phospholipid of alveolar surfactant ( ,   -  ).	transcription
69667	3	336219	5	NULL	NULL	0	NULL	PtdCho	Chemical		is					phosphatidylcholine	Chemical				NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_15	15772421	Ceramide potently induces programmed cell death in lung cells and inhibits the biosynthesis of phosphatidylcholine (PtdCho), the predominant phospholipid of alveolar surfactant ( ,   -  ).	transcription
69668	4	336219	5	NULL	NULL	0	NULL	PtdCho	Chemical		is a type of					phospholipid	Chemical				NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_15	15772421	Ceramide potently induces programmed cell death in lung cells and inhibits the biosynthesis of phosphatidylcholine (PtdCho), the predominant phospholipid of alveolar surfactant ( ,   -  ).	transcription
69669	5	336219	5	NULL	NULL	0	NULL	PtdCho	Chemical		is predominant in					alveolar surfactant	Chemical				NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_15	15772421	Ceramide potently induces programmed cell death in lung cells and inhibits the biosynthesis of phosphatidylcholine (PtdCho), the predominant phospholipid of alveolar surfactant ( ,   -  ).	transcription
71720	1	336219	7	NULL	NULL	0	NULL	Ceramide	Chemical		induce		potently			programmed cell death	Process				NULL	lung cells	0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_15	15772421	Ceramide potently induces programmed cell death in lung cells and inhibits the biosynthesis of phosphatidylcholine (PtdCho), the predominant phospholipid of alveolar surfactant ( ,   -  ).	transcription
71721	2	336219	7	NULL	NULL	0	NULL	ceramide	Chemical		inhibit					PtdCho	Chemical	biosynthesis of			NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_15	15772421	Ceramide potently induces programmed cell death in lung cells and inhibits the biosynthesis of phosphatidylcholine (PtdCho), the predominant phospholipid of alveolar surfactant ( ,   -  ).	transcription
71722	3	336219	7	NULL	NULL	0	NULL	PtdCho	Chemical		is					phosphatidylcholine	Chemical				NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_15	15772421	Ceramide potently induces programmed cell death in lung cells and inhibits the biosynthesis of phosphatidylcholine (PtdCho), the predominant phospholipid of alveolar surfactant ( ,   -  ).	transcription
71723	4	336219	7	NULL	NULL	0	NULL	phosphatidylcholine	Chemical		phospholipid of		predominant			alveolar surfactant	Chemical				NULL		0	NULL	NULL	NULL	gw70_jlipidres_46_6_1229_s_15	15772421	Ceramide potently induces programmed cell death in lung cells and inhibits the biosynthesis of phosphatidylcholine (PtdCho), the predominant phospholipid of alveolar surfactant ( ,   -  ).	transcription
69670	1	336221	5	NULL	NULL	NULL	NULL	apoptosis	Process		is induced by					Choline	Chemical	deficiency of			NULL	PC12 cells	NULL	NULL	NULL	NULL	gw60_neuroscience_118_1_107_s_341	12676142	Choline deficiency-induced apoptosis in PC12 cells is associated with diminished membrane phosphatidylcholine and sphingomyelin, accumulation of ceramide and diacylglycerol, and activation of a caspase.	transcription
69671	2	336221	5	NULL	NULL	NULL	NULL	statement 1	Process		is associated with					phosphatidylcholine	Chemical	diminished;;membrane			NULL	PC12 cells	NULL	NULL	NULL	NULL	gw60_neuroscience_118_1_107_s_341	12676142	Choline deficiency-induced apoptosis in PC12 cells is associated with diminished membrane phosphatidylcholine and sphingomyelin, accumulation of ceramide and diacylglycerol, and activation of a caspase.	transcription
69672	3	336221	5	NULL	NULL	NULL	NULL	statement 1	Process		is associated with					sphingomyelin	Chemical	diminished;;membrane			NULL	PC12 cells	NULL	NULL	NULL	NULL	gw60_neuroscience_118_1_107_s_341	12676142	Choline deficiency-induced apoptosis in PC12 cells is associated with diminished membrane phosphatidylcholine and sphingomyelin, accumulation of ceramide and diacylglycerol, and activation of a caspase.	transcription
69673	4	336221	5	NULL	NULL	0	NULL	statement 1	Process		is associated with					ceramide	Chemical	accumulation of			NULL	PC12 cells	0	NULL	NULL	NULL	gw60_neuroscience_118_1_107_s_341	12676142	Choline deficiency-induced apoptosis in PC12 cells is associated with diminished membrane phosphatidylcholine and sphingomyelin, accumulation of ceramide and diacylglycerol, and activation of a caspase.	transcription
69674	5	336221	5	NULL	NULL	NULL	NULL	statement 1	Process		is associated with					diacylglycerol	Chemical	accumulation of			NULL	PC12 cells	NULL	NULL	NULL	NULL	gw60_neuroscience_118_1_107_s_341	12676142	Choline deficiency-induced apoptosis in PC12 cells is associated with diminished membrane phosphatidylcholine and sphingomyelin, accumulation of ceramide and diacylglycerol, and activation of a caspase.	transcription
69675	6	336221	5	NULL	NULL	0	NULL	statement 1	Process		is associated with					caspase	GP	activation of			NULL	PC12 cells	0	NULL	NULL	NULL	gw60_neuroscience_118_1_107_s_341	12676142	Choline deficiency-induced apoptosis in PC12 cells is associated with diminished membrane phosphatidylcholine and sphingomyelin, accumulation of ceramide and diacylglycerol, and activation of a caspase.	transcription
71724	1	336221	7	NULL	NULL	0	NULL	Choline	Chemical	deficiency of	induce					apoptosis	Process				NULL	PC12 cells	0	NULL	NULL	NULL	gw60_neuroscience_118_1_107_s_341	12676142	Choline deficiency-induced apoptosis in PC12 cells is associated with diminished membrane phosphatidylcholine and sphingomyelin, accumulation of ceramide and diacylglycerol, and activation of a caspase.	transcription
71725	2	336221	7	NULL	NULL	0	NULL	statement 1	Process		is associated with					phosphatidylcholine 	Chemical	diminished membrane			NULL		0	NULL	NULL	NULL	gw60_neuroscience_118_1_107_s_341	12676142	Choline deficiency-induced apoptosis in PC12 cells is associated with diminished membrane phosphatidylcholine and sphingomyelin, accumulation of ceramide and diacylglycerol, and activation of a caspase.	transcription
71726	3	336221	7	NULL	NULL	0	NULL	statement 1	Process		is associated with					 sphingomyelin	Chemical				NULL		0	NULL	NULL	NULL	gw60_neuroscience_118_1_107_s_341	12676142	Choline deficiency-induced apoptosis in PC12 cells is associated with diminished membrane phosphatidylcholine and sphingomyelin, accumulation of ceramide and diacylglycerol, and activation of a caspase.	transcription
71727	4	336221	7	NULL	NULL	0	NULL	statement 1	Process		is associated with					ceramide	Chemical	accumulation of			NULL		0	NULL	NULL	NULL	gw60_neuroscience_118_1_107_s_341	12676142	Choline deficiency-induced apoptosis in PC12 cells is associated with diminished membrane phosphatidylcholine and sphingomyelin, accumulation of ceramide and diacylglycerol, and activation of a caspase.	transcription
71728	5	336221	7	NULL	NULL	NULL	NULL	statement 1	Process		associated with					diacylglycerol	Chemical	accumulation of			NULL		NULL	NULL	NULL	NULL	gw60_neuroscience_118_1_107_s_341	12676142	Choline deficiency-induced apoptosis in PC12 cells is associated with diminished membrane phosphatidylcholine and sphingomyelin, accumulation of ceramide and diacylglycerol, and activation of a caspase.	transcription
71729	6	336221	7	NULL	NULL	0	NULL	statement 1	Process		is associated with					caspase	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_neuroscience_118_1_107_s_341	12676142	Choline deficiency-induced apoptosis in PC12 cells is associated with diminished membrane phosphatidylcholine and sphingomyelin, accumulation of ceramide and diacylglycerol, and activation of a caspase.	transcription
69676	1	336222	5	NULL	NULL	0	NULL	sphingomyelin	Chemical	hydrolysis of	forms					ceramide	Chemical	biologically active;;intracellular			NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_5_815_s_3	11971953	They catalyze the hydrolysis of sphingomyelin, giving rise to the intracellular formation of biologically active ceramide and phosphatidylcholine.	transcription
69677	2	336222	5	NULL	NULL	0	NULL	sphingomyelin	Chemical	hydrolysis of	forms					phosphatidylcholine	Chemical	biologically active;;intracellular			NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_5_815_s_3	11971953	They catalyze the hydrolysis of sphingomyelin, giving rise to the intracellular formation of biologically active ceramide and phosphatidylcholine.	transcription
71730	1	336222	7	NULL	NULL	NULL	NULL	sphingomyelin	Chemical		hydrolyzed to					ceramide	Chemical	 intracellular formation of biologically active			NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_43_5_815_s_3	11971953	They catalyze the hydrolysis of sphingomyelin, giving rise to the intracellular formation of biologically active ceramide and phosphatidylcholine.	transcription
71731	2	336222	7	NULL	NULL	0	NULL	sphingomyelin	Chemical		hydrolyzed to					phosphatidylcholine	Chemical	 intracellular formation of biologically active			NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_5_815_s_3	11971953	They catalyze the hydrolysis of sphingomyelin, giving rise to the intracellular formation of biologically active ceramide and phosphatidylcholine.	transcription
71934	1	336223	7	NULL	NULL	NULL	NULL	sphingomyelinases	GP		hydrolyze					sphingomyelin	Chemical				NULL	intact cells	NULL	NULL	NULL	NULL	gw60_jlipidres_43_5_815_s_79	11971953	Determination of SMase-activity   phingomyelinases in intact cells hydrolyze sphingomyelin leading to the formation of ceramide and phosphatidylcholine ( 23).	transcription
71935	2	336223	7	NULL	NULL	0	NULL	statement 1	Process		forms					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jlipidres_43_5_815_s_79	11971953	Determination of SMase-activity   phingomyelinases in intact cells hydrolyze sphingomyelin leading to the formation of ceramide and phosphatidylcholine ( 23).	transcription
71936	3	336223	7	NULL	NULL	NULL	NULL	statement 1	Process		forms					phosphatidylcholine	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_jlipidres_43_5_815_s_79	11971953	Determination of SMase-activity   phingomyelinases in intact cells hydrolyze sphingomyelin leading to the formation of ceramide and phosphatidylcholine ( 23).	transcription
71937	1	336224	7	NULL	NULL	0	NULL	SMS	GP		catalyze					sphingomyelin	Chemical	production of			NULL		0	NULL	NULL	NULL	gw70_gene_363_0_123_s_173	16226406	SMS catalyzes the production of sphingomyelin and diacylglycerol (DAG) using ceramide  and phosphatidylcholine as substrates (  Hannun et al., 2001 and   Hannun and Luberto, 2004).	transcription
71938	2	336224	7	NULL	NULL	0	NULL	SMS	GP		catalyze					DAG	Chemical	production of			NULL		0	NULL	NULL	NULL	gw70_gene_363_0_123_s_173	16226406	SMS catalyzes the production of sphingomyelin and diacylglycerol (DAG) using ceramide  and phosphatidylcholine as substrates (  Hannun et al., 2001 and   Hannun and Luberto, 2004).	transcription
71939	3	336224	7	NULL	NULL	0	NULL	ceramide	Chemical		substrate for					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_gene_363_0_123_s_173	16226406	SMS catalyzes the production of sphingomyelin and diacylglycerol (DAG) using ceramide  and phosphatidylcholine as substrates (  Hannun et al., 2001 and   Hannun and Luberto, 2004).	transcription
71940	4	336224	7	NULL	NULL	0	NULL	ceramide	Chemical		substrate for					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_gene_363_0_123_s_173	16226406	SMS catalyzes the production of sphingomyelin and diacylglycerol (DAG) using ceramide  and phosphatidylcholine as substrates (  Hannun et al., 2001 and   Hannun and Luberto, 2004).	transcription
71941	5	336224	7	NULL	NULL	0	NULL	phosphatidylcholine	Chemical		substrate for					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_gene_363_0_123_s_173	16226406	SMS catalyzes the production of sphingomyelin and diacylglycerol (DAG) using ceramide  and phosphatidylcholine as substrates (  Hannun et al., 2001 and   Hannun and Luberto, 2004).	transcription
71942	6	336224	7	NULL	NULL	0	NULL	phosphatidylcholine	Chemical		substrate for					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_gene_363_0_123_s_173	16226406	SMS catalyzes the production of sphingomyelin and diacylglycerol (DAG) using ceramide  and phosphatidylcholine as substrates (  Hannun et al., 2001 and   Hannun and Luberto, 2004).	transcription
71943	7	336224	7	NULL	NULL	0	NULL	DAG	Chemical		is					diacylglycerol	Chemical				NULL		0	NULL	NULL	NULL	gw70_gene_363_0_123_s_173	16226406	SMS catalyzes the production of sphingomyelin and diacylglycerol (DAG) using ceramide  and phosphatidylcholine as substrates (  Hannun et al., 2001 and   Hannun and Luberto, 2004).	transcription
71944	1	336225	7	NULL	NULL	NULL	NULL	phospholipase C	GP		mediate					PC	Chemical	hydrolysis of;;membrane			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_43_27800_s_20	9774389	Second messengers such as diacylglycerol and ceramide are generated in part by phospholipase C- and sphingomyelinase-mediated hydrolysis of membrane phosphatidylcholine (PC) and sphingomyelin (SM), respectively.	transcription
71945	2	336225	7	NULL	NULL	0	NULL	sphingomyelinase	GP		mediate					SM	Chemical	hydrolysis of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_43_27800_s_20	9774389	Second messengers such as diacylglycerol and ceramide are generated in part by phospholipase C- and sphingomyelinase-mediated hydrolysis of membrane phosphatidylcholine (PC) and sphingomyelin (SM), respectively.	transcription
71946	3	336225	7	NULL	NULL	0	NULL	statement 1	Process		generate					diacylglycerol	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_43_27800_s_20	9774389	Second messengers such as diacylglycerol and ceramide are generated in part by phospholipase C- and sphingomyelinase-mediated hydrolysis of membrane phosphatidylcholine (PC) and sphingomyelin (SM), respectively.	transcription
71947	4	336225	7	NULL	NULL	0	NULL	statement 1	Process		generate					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_43_27800_s_20	9774389	Second messengers such as diacylglycerol and ceramide are generated in part by phospholipase C- and sphingomyelinase-mediated hydrolysis of membrane phosphatidylcholine (PC) and sphingomyelin (SM), respectively.	transcription
71948	5	336225	7	NULL	NULL	0	NULL	PC	Chemical		is					phosphatidylcholine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_43_27800_s_20	9774389	Second messengers such as diacylglycerol and ceramide are generated in part by phospholipase C- and sphingomyelinase-mediated hydrolysis of membrane phosphatidylcholine (PC) and sphingomyelin (SM), respectively.	transcription
71949	6	336225	7	NULL	NULL	0	NULL	SM	Chemical		is					sphingomyelin	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_43_27800_s_20	9774389	Second messengers such as diacylglycerol and ceramide are generated in part by phospholipase C- and sphingomyelinase-mediated hydrolysis of membrane phosphatidylcholine (PC) and sphingomyelin (SM), respectively.	transcription
71950	7	336225	7	NULL	NULL	0	NULL	diacylglycerol	Chemical		is a type of					secondary messenger	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_43_27800_s_20	9774389	Second messengers such as diacylglycerol and ceramide are generated in part by phospholipase C- and sphingomyelinase-mediated hydrolysis of membrane phosphatidylcholine (PC) and sphingomyelin (SM), respectively.	transcription
71951	1	336226	7	NULL	NULL	NULL	NULL	sphingomyelin	Chemical	appearance of	shows					serine ceramide pathway	Process	increase in synthetic activity of			NULL	fa/fa islets	NULL	NULL	NULL	NULL	gw60_jbiolchem_273_49_32487_s_81	9829981	The appearance of [3]sphingomyelin, [3]phosphatidylethanolamine, and [3]phosphatidylcholine were the same in  +/+ and  fa/fa islets, evidence that the increase in synthetic activity was limited to the serine   ceramide pathway.	transcription
71952	2	336226	7	NULL	NULL	0	NULL	phosphatidylethanolamine	Chemical	appearance of	shows					serine ceramide pathway	Process	increase in synthetic activity of			NULL	fa/fa islets	0	NULL	NULL	NULL	gw60_jbiolchem_273_49_32487_s_81	9829981	The appearance of [3]sphingomyelin, [3]phosphatidylethanolamine, and [3]phosphatidylcholine were the same in  +/+ and  fa/fa islets, evidence that the increase in synthetic activity was limited to the serine   ceramide pathway.	transcription
71953	3	336226	7	NULL	NULL	0	NULL	phosphatidylcholine	Chemical	appearance of	shows					serine ceramide pathway	Process	increase in synthetic activity of			NULL	fa/fa islets	0	NULL	NULL	NULL	gw60_jbiolchem_273_49_32487_s_81	9829981	The appearance of [3]sphingomyelin, [3]phosphatidylethanolamine, and [3]phosphatidylcholine were the same in  +/+ and  fa/fa islets, evidence that the increase in synthetic activity was limited to the serine   ceramide pathway.	transcription
71954	1	336227	7	NULL	NULL	0	NULL	LPS	Chemical		induce					TLR4	GP	assembly of			NULL		0	NULL	NULL	NULL	abs-batch0740-0759_j-leukoc-biol_80_2_16754725_s_4	16754725	The purpose of this study is to determine if  LPS-induced TLR4 assembly and activation are dependent on the sphingolipid  metabolite ceramide produced by phosphatidylcholine-specific phospholipase  C (PC-PLC) or CD14.	transcription
71955	2	336227	7	NULL	NULL	0	NULL	LPS	Chemical		induce					TLR4	GP	activation of			NULL		0	NULL	NULL	NULL	abs-batch0740-0759_j-leukoc-biol_80_2_16754725_s_4	16754725	The purpose of this study is to determine if  LPS-induced TLR4 assembly and activation are dependent on the sphingolipid  metabolite ceramide produced by phosphatidylcholine-specific phospholipase  C (PC-PLC) or CD14.	transcription
72116	3	336227	7	NULL	NULL	0	NULL	PC-PLC	GP		produce					ceramide	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_j-leukoc-biol_80_2_16754725_s_4	16754725	The purpose of this study is to determine if  LPS-induced TLR4 assembly and activation are dependent on the sphingolipid  metabolite ceramide produced by phosphatidylcholine-specific phospholipase  C (PC-PLC) or CD14.	transcription
72117	4	336227	7	NULL	NULL	0	NULL	CD14	GP		produce					ceramide	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_j-leukoc-biol_80_2_16754725_s_4	16754725	The purpose of this study is to determine if  LPS-induced TLR4 assembly and activation are dependent on the sphingolipid  metabolite ceramide produced by phosphatidylcholine-specific phospholipase  C (PC-PLC) or CD14.	transcription
72118	5	336227	7	NULL	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_j-leukoc-biol_80_2_16754725_s_4	16754725	The purpose of this study is to determine if  LPS-induced TLR4 assembly and activation are dependent on the sphingolipid  metabolite ceramide produced by phosphatidylcholine-specific phospholipase  C (PC-PLC) or CD14.	transcription
72119	6	336227	7	NULL	NULL	0	NULL	PC-PLC	GP		is					phosphatidylcholine-specific phospholipase C	GP				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_j-leukoc-biol_80_2_16754725_s_4	16754725	The purpose of this study is to determine if  LPS-induced TLR4 assembly and activation are dependent on the sphingolipid  metabolite ceramide produced by phosphatidylcholine-specific phospholipase  C (PC-PLC) or CD14.	transcription
72120	7	336227	7	NULL	NULL	0	NULL	ceramide	Chemical		is a type of					sphingolipid metabolite	Chemical				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_j-leukoc-biol_80_2_16754725_s_4	16754725	The purpose of this study is to determine if  LPS-induced TLR4 assembly and activation are dependent on the sphingolipid  metabolite ceramide produced by phosphatidylcholine-specific phospholipase  C (PC-PLC) or CD14.	transcription
72121	1	336228	7	NULL	NULL	0	NULL	MAb90	GP		induce					ceramide	Chemical	production of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_5060_s_79	9478956	MAb90 and YTH862 Induce Ceramide Production under the Control of a Phosphatidylcholine-specific Phospholipase C-- Okadaic acid has been reported to inhibit ceramide-induced apoptosis, possibly by blocking a ceramide-activated protein phosphatase which belongs to the heterodimeric subfamily of the phosphatases 2A group ( 40).	transcription
72122	2	336228	7	NULL	NULL	0	NULL	YTH862	GP		induce					ceramide	Chemical	production of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_5060_s_79	9478956	MAb90 and YTH862 Induce Ceramide Production under the Control of a Phosphatidylcholine-specific Phospholipase C-- Okadaic acid has been reported to inhibit ceramide-induced apoptosis, possibly by blocking a ceramide-activated protein phosphatase which belongs to the heterodimeric subfamily of the phosphatases 2A group ( 40).	transcription
72123	3	336228	7	NULL	NULL	0	NULL	statement 1	Process		under the control of					Phosphatidylcholine-specific Phospholipase C	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_5060_s_79	9478956	MAb90 and YTH862 Induce Ceramide Production under the Control of a Phosphatidylcholine-specific Phospholipase C-- Okadaic acid has been reported to inhibit ceramide-induced apoptosis, possibly by blocking a ceramide-activated protein phosphatase which belongs to the heterodimeric subfamily of the phosphatases 2A group ( 40).	transcription
72124	4	336228	7	NULL	NULL	0	NULL	statement 2	Process		under the control of					phosphatidylcholine-specific phospholipase C	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_5060_s_79	9478956	MAb90 and YTH862 Induce Ceramide Production under the Control of a Phosphatidylcholine-specific Phospholipase C-- Okadaic acid has been reported to inhibit ceramide-induced apoptosis, possibly by blocking a ceramide-activated protein phosphatase which belongs to the heterodimeric subfamily of the phosphatases 2A group ( 40).	transcription
72125	5	336228	7	NULL	NULL	0	NULL	ceramide	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_5060_s_79	9478956	MAb90 and YTH862 Induce Ceramide Production under the Control of a Phosphatidylcholine-specific Phospholipase C-- Okadaic acid has been reported to inhibit ceramide-induced apoptosis, possibly by blocking a ceramide-activated protein phosphatase which belongs to the heterodimeric subfamily of the phosphatases 2A group ( 40).	transcription
72126	6	336228	7	NULL	NULL	0	NULL	Okadaic acid	Chemical		inhibit					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_5060_s_79	9478956	MAb90 and YTH862 Induce Ceramide Production under the Control of a Phosphatidylcholine-specific Phospholipase C-- Okadaic acid has been reported to inhibit ceramide-induced apoptosis, possibly by blocking a ceramide-activated protein phosphatase which belongs to the heterodimeric subfamily of the phosphatases 2A group ( 40).	transcription
72127	7	336228	7	NULL	NULL	0	NULL	statement 6	Process		occur		possibly			ceramide-activated protein phosphatase	GP	by blocking of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_5060_s_79	9478956	MAb90 and YTH862 Induce Ceramide Production under the Control of a Phosphatidylcholine-specific Phospholipase C-- Okadaic acid has been reported to inhibit ceramide-induced apoptosis, possibly by blocking a ceramide-activated protein phosphatase which belongs to the heterodimeric subfamily of the phosphatases 2A group ( 40).	transcription
72128	8	336228	7	NULL	NULL	0	NULL	ceramide-activated protein phosphatase	GP		belongs to					phosphatases 2A group	GP	heterodimeric subfamily of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_5060_s_79	9478956	MAb90 and YTH862 Induce Ceramide Production under the Control of a Phosphatidylcholine-specific Phospholipase C-- Okadaic acid has been reported to inhibit ceramide-induced apoptosis, possibly by blocking a ceramide-activated protein phosphatase which belongs to the heterodimeric subfamily of the phosphatases 2A group ( 40).	transcription
72129	1	336229	7	NULL	NULL	0	NULL	TNF 	GP		interacts with					TNF receptor	GP				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_14_0_649_s_387	8717528	According to the current model, the interaction of TNF with  the 55-kDa TNF receptor activates an acidic sphingomyelinase (Smase) through the  generation of diacylglycerol by a phosphatidylcholine-specific phospholipase C. Smase  leads to the production of ceramide.	transcription
72130	2	336229	7	NULL	NULL	0	NULL	statement 1	Process		activates an					Smase	GP	acidic			NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_14_0_649_s_387	8717528	According to the current model, the interaction of TNF with  the 55-kDa TNF receptor activates an acidic sphingomyelinase (Smase) through the  generation of diacylglycerol by a phosphatidylcholine-specific phospholipase C. Smase  leads to the production of ceramide.	transcription
72131	3	336229	7	NULL	NULL	0	NULL	phosphatidylcholine-specific phospholipase C	GP		generates					diacylglycerol	Chemical				NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_14_0_649_s_387	8717528	According to the current model, the interaction of TNF with  the 55-kDa TNF receptor activates an acidic sphingomyelinase (Smase) through the  generation of diacylglycerol by a phosphatidylcholine-specific phospholipase C. Smase  leads to the production of ceramide.	transcription
72132	4	336229	7	NULL	NULL	0	NULL	statement 2	Process		occur through					diacylglycerol	Chemical	generation of			NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_14_0_649_s_387	8717528	According to the current model, the interaction of TNF with  the 55-kDa TNF receptor activates an acidic sphingomyelinase (Smase) through the  generation of diacylglycerol by a phosphatidylcholine-specific phospholipase C. Smase  leads to the production of ceramide.	transcription
72133	5	336229	7	NULL	NULL	0	NULL	Smase	GP		leads to					ceramide	Chemical	production of			NULL		0	NULL	NULL	NULL	gw70_annurevimmunol_14_0_649_s_387	8717528	According to the current model, the interaction of TNF with  the 55-kDa TNF receptor activates an acidic sphingomyelinase (Smase) through the  generation of diacylglycerol by a phosphatidylcholine-specific phospholipase C. Smase  leads to the production of ceramide.	transcription
72134	1	336230	7	NULL	NULL	0	NULL	 Choline	Chemical	deficiency of	induce					apoptosis	Process				NULL	PC12 cells 	0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_87_s_483	12531541	C.L. Yen, M.H. Mar and S.H. Zeisel , Choline deficiency-induced apoptosis in PC12 cells is associated with diminished membrane phosphatidylcholine and sphingomyelin, accumulation of ceramide and diacylglycerol, and activation of a caspase.	transcription
72135	2	336230	7	NULL	NULL	0	NULL	statement 1	Process		associated with					phosphatidylcholine	Chemical	diminished;; membrane			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_87_s_483	12531541	C.L. Yen, M.H. Mar and S.H. Zeisel , Choline deficiency-induced apoptosis in PC12 cells is associated with diminished membrane phosphatidylcholine and sphingomyelin, accumulation of ceramide and diacylglycerol, and activation of a caspase.	transcription
72136	3	336230	7	NULL	NULL	0	NULL	statement 1	Process		associated with					sphingomyelin	Chemical	diminished;; membrane			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_87_s_483	12531541	C.L. Yen, M.H. Mar and S.H. Zeisel , Choline deficiency-induced apoptosis in PC12 cells is associated with diminished membrane phosphatidylcholine and sphingomyelin, accumulation of ceramide and diacylglycerol, and activation of a caspase.	transcription
72137	4	336230	7	NULL	NULL	0	NULL	statement 1	Process		associated with					ceramide	Chemical	accumulation of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_87_s_483	12531541	C.L. Yen, M.H. Mar and S.H. Zeisel , Choline deficiency-induced apoptosis in PC12 cells is associated with diminished membrane phosphatidylcholine and sphingomyelin, accumulation of ceramide and diacylglycerol, and activation of a caspase.	transcription
72138	5	336230	7	NULL	NULL	0	NULL	statement 1	Process		associated with					diacylglycerol	Chemical	accumulation of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_87_s_483	12531541	C.L. Yen, M.H. Mar and S.H. Zeisel , Choline deficiency-induced apoptosis in PC12 cells is associated with diminished membrane phosphatidylcholine and sphingomyelin, accumulation of ceramide and diacylglycerol, and activation of a caspase.	transcription
72139	6	336230	7	NULL	NULL	0	NULL	statement 1	Process		associated with					caspase	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1585_2_87_s_483	12531541	C.L. Yen, M.H. Mar and S.H. Zeisel , Choline deficiency-induced apoptosis in PC12 cells is associated with diminished membrane phosphatidylcholine and sphingomyelin, accumulation of ceramide and diacylglycerol, and activation of a caspase.	transcription
72147	1	336231	7	NULL	NULL	NULL	NULL	N. gonorrhoeae	Organism		activates					PC-PLC	GP				NULL	 human epithelial cells	NULL	NULL	NULL	NULL	gw60_cell_91_5_605_s_3	9393854	Using different human  epithelial cells and primary fibroblasts, we show here an activation of the phosphatidylcholine-specific  phospholipase C (PC-PLC) and acidic sphingomyelinase (ASM) by N. gonorrhoeae, resulting in the release of diacylglycerol  and ceramide.	transcription
72148	2	336231	7	NULL	NULL	NULL	NULL	N. gonorrhoeae	Organism		activates 					ASM	GP				NULL	 human epithelial cells	NULL	NULL	NULL	NULL	gw60_cell_91_5_605_s_3	9393854	Using different human  epithelial cells and primary fibroblasts, we show here an activation of the phosphatidylcholine-specific  phospholipase C (PC-PLC) and acidic sphingomyelinase (ASM) by N. gonorrhoeae, resulting in the release of diacylglycerol  and ceramide.	transcription
72149	3	336231	7	NULL	NULL	0	NULL	N. gonorrhoeae	Organism		activates					PC-PLC	GP				NULL	primary fibroblasts	0	NULL	NULL	NULL	gw60_cell_91_5_605_s_3	9393854	Using different human  epithelial cells and primary fibroblasts, we show here an activation of the phosphatidylcholine-specific  phospholipase C (PC-PLC) and acidic sphingomyelinase (ASM) by N. gonorrhoeae, resulting in the release of diacylglycerol  and ceramide.	transcription
72150	4	336231	7	NULL	NULL	NULL	NULL	N. gonorrhoeae	Organism		activates					ASM	GP				NULL	primary fibroblasts	NULL	NULL	NULL	NULL	gw60_cell_91_5_605_s_3	9393854	Using different human  epithelial cells and primary fibroblasts, we show here an activation of the phosphatidylcholine-specific  phospholipase C (PC-PLC) and acidic sphingomyelinase (ASM) by N. gonorrhoeae, resulting in the release of diacylglycerol  and ceramide.	transcription
72151	5	336231	7	NULL	NULL	0	NULL	statement 1	Process		result in					diacylglycerol	Chemical	release of			NULL		0	NULL	NULL	NULL	gw60_cell_91_5_605_s_3	9393854	Using different human  epithelial cells and primary fibroblasts, we show here an activation of the phosphatidylcholine-specific  phospholipase C (PC-PLC) and acidic sphingomyelinase (ASM) by N. gonorrhoeae, resulting in the release of diacylglycerol  and ceramide.	transcription
72152	6	336231	7	NULL	NULL	0	NULL	statement 2	Process		result in					diacylglycerol	Chemical	release of			NULL		0	NULL	NULL	NULL	gw60_cell_91_5_605_s_3	9393854	Using different human  epithelial cells and primary fibroblasts, we show here an activation of the phosphatidylcholine-specific  phospholipase C (PC-PLC) and acidic sphingomyelinase (ASM) by N. gonorrhoeae, resulting in the release of diacylglycerol  and ceramide.	transcription
72153	7	336231	7	NULL	NULL	0	NULL	statement 3	Process		result in					diacylglycerol	Chemical	release of			NULL		0	NULL	NULL	NULL	gw60_cell_91_5_605_s_3	9393854	Using different human  epithelial cells and primary fibroblasts, we show here an activation of the phosphatidylcholine-specific  phospholipase C (PC-PLC) and acidic sphingomyelinase (ASM) by N. gonorrhoeae, resulting in the release of diacylglycerol  and ceramide.	transcription
72154	8	336231	7	NULL	NULL	0	NULL	statement 4	Process		result in					diacylglycerol	Chemical	release of			NULL		0	NULL	NULL	NULL	gw60_cell_91_5_605_s_3	9393854	Using different human  epithelial cells and primary fibroblasts, we show here an activation of the phosphatidylcholine-specific  phospholipase C (PC-PLC) and acidic sphingomyelinase (ASM) by N. gonorrhoeae, resulting in the release of diacylglycerol  and ceramide.	transcription
72155	9	336231	7	NULL	NULL	0	NULL	statement 1	Process		result in					ceramide	Chemical	release of			NULL		0	NULL	NULL	NULL	gw60_cell_91_5_605_s_3	9393854	Using different human  epithelial cells and primary fibroblasts, we show here an activation of the phosphatidylcholine-specific  phospholipase C (PC-PLC) and acidic sphingomyelinase (ASM) by N. gonorrhoeae, resulting in the release of diacylglycerol  and ceramide.	transcription
72156	10	336231	7	NULL	NULL	0	NULL	statement 2	Process		result in					ceramide	Chemical	release of			NULL		0	NULL	NULL	NULL	gw60_cell_91_5_605_s_3	9393854	Using different human  epithelial cells and primary fibroblasts, we show here an activation of the phosphatidylcholine-specific  phospholipase C (PC-PLC) and acidic sphingomyelinase (ASM) by N. gonorrhoeae, resulting in the release of diacylglycerol  and ceramide.	transcription
72157	11	336231	7	NULL	NULL	0	NULL	statement 3	Process		result in					ceramide	Chemical	release of			NULL		0	NULL	NULL	NULL	gw60_cell_91_5_605_s_3	9393854	Using different human  epithelial cells and primary fibroblasts, we show here an activation of the phosphatidylcholine-specific  phospholipase C (PC-PLC) and acidic sphingomyelinase (ASM) by N. gonorrhoeae, resulting in the release of diacylglycerol  and ceramide.	transcription
72158	12	336231	7	NULL	NULL	0	NULL	statement 4	Process		result in					ceramide	Chemical	release of			NULL		0	NULL	NULL	NULL	gw60_cell_91_5_605_s_3	9393854	Using different human  epithelial cells and primary fibroblasts, we show here an activation of the phosphatidylcholine-specific  phospholipase C (PC-PLC) and acidic sphingomyelinase (ASM) by N. gonorrhoeae, resulting in the release of diacylglycerol  and ceramide.	transcription
72159	13	336231	7	NULL	NULL	0	NULL	PC-PLC	GP		is					phosphatidylcholine-specific phospholipase C	GP				NULL		0	NULL	NULL	NULL	gw60_cell_91_5_605_s_3	9393854	Using different human  epithelial cells and primary fibroblasts, we show here an activation of the phosphatidylcholine-specific  phospholipase C (PC-PLC) and acidic sphingomyelinase (ASM) by N. gonorrhoeae, resulting in the release of diacylglycerol  and ceramide.	transcription
72160	14	336231	7	NULL	NULL	0	NULL	ASM	GP		is					acidic sphingomyelinase	GP				NULL		0	NULL	NULL	NULL	gw60_cell_91_5_605_s_3	9393854	Using different human  epithelial cells and primary fibroblasts, we show here an activation of the phosphatidylcholine-specific  phospholipase C (PC-PLC) and acidic sphingomyelinase (ASM) by N. gonorrhoeae, resulting in the release of diacylglycerol  and ceramide.	transcription
72161	1	336232	7	NULL	NULL	0	NULL	TNF-R55	GP		initiates		sequentially	C-terminal domain		phosphatidylcholine-specific phospholipase C	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_cell_86_6_937_s_12	8808629	Recent studies have identified a C-terminal domain  of TNF-R55 that sequentially initiates the activation of a phosphatidylcholine-specific phospholipase C  and an acidic sphingomyelinase (A-SMase), generating ceramide (Schutze et al., 1992   ;  Wiegmann  et al., 1994   ).	transcription
72162	2	336232	7	NULL	NULL	NULL	NULL	TNF-R55	GP		initiates		sequentially	C-terminal domain		ASMase	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_cell_86_6_937_s_12	8808629	Recent studies have identified a C-terminal domain  of TNF-R55 that sequentially initiates the activation of a phosphatidylcholine-specific phospholipase C  and an acidic sphingomyelinase (A-SMase), generating ceramide (Schutze et al., 1992   ;  Wiegmann  et al., 1994   ).	transcription
72163	3	336232	7	NULL	NULL	0	NULL	statement 1	Process		generate					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_cell_86_6_937_s_12	8808629	Recent studies have identified a C-terminal domain  of TNF-R55 that sequentially initiates the activation of a phosphatidylcholine-specific phospholipase C  and an acidic sphingomyelinase (A-SMase), generating ceramide (Schutze et al., 1992   ;  Wiegmann  et al., 1994   ).	transcription
72164	4	336232	7	NULL	NULL	0	NULL	statement 2	Process		generate					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_cell_86_6_937_s_12	8808629	Recent studies have identified a C-terminal domain  of TNF-R55 that sequentially initiates the activation of a phosphatidylcholine-specific phospholipase C  and an acidic sphingomyelinase (A-SMase), generating ceramide (Schutze et al., 1992   ;  Wiegmann  et al., 1994   ).	transcription
72165	5	336232	7	NULL	NULL	0	NULL	ASMase	GP		is					acidic sphingomyelinase	GP				NULL		0	NULL	NULL	NULL	gw60_cell_86_6_937_s_12	8808629	Recent studies have identified a C-terminal domain  of TNF-R55 that sequentially initiates the activation of a phosphatidylcholine-specific phospholipase C  and an acidic sphingomyelinase (A-SMase), generating ceramide (Schutze et al., 1992   ;  Wiegmann  et al., 1994   ).	transcription
72366	1	336234	7	NULL	NULL	NULL	NULL	phosphatidylcholine specific phospholipase	GP	stimulation of	results in					diacylglycerol	Chemical	generation of			NULL	epithelial cell lines	NULL	NULL	NULL	NULL	gw60_microbesinfect_2_7_821_s_27	10955963	Into some epithelial cell lines (e.g., Chang cells), this entry process involves a signaling pathway requiring stimulation of the phosphatidylcholine specific phospholipase and acidic sphingomyelinase which results in the generation of the second messagers diacylglycerol and ceramide, respectively [  8.	transcription
72367	2	336234	7	NULL	NULL	NULL	NULL	acidic sphingomyelinase	GP		results in					ceramide	Chemical	generation of			NULL	epithelial cell lines	NULL	NULL	NULL	NULL	gw60_microbesinfect_2_7_821_s_27	10955963	Into some epithelial cell lines (e.g., Chang cells), this entry process involves a signaling pathway requiring stimulation of the phosphatidylcholine specific phospholipase and acidic sphingomyelinase which results in the generation of the second messagers diacylglycerol and ceramide, respectively [  8.	transcription
72368	3	336234	7	NULL	NULL	NULL	NULL	diacylglycerol	Chemical		is a type of					second messagers	Chemical				NULL		NULL	NULL	NULL	NULL	gw60_microbesinfect_2_7_821_s_27	10955963	Into some epithelial cell lines (e.g., Chang cells), this entry process involves a signaling pathway requiring stimulation of the phosphatidylcholine specific phospholipase and acidic sphingomyelinase which results in the generation of the second messagers diacylglycerol and ceramide, respectively [  8.	transcription
72369	4	336234	7	NULL	NULL	0	NULL	ceramide	Chemical		is a type of					second messagers	Chemical				NULL		0	NULL	NULL	NULL	gw60_microbesinfect_2_7_821_s_27	10955963	Into some epithelial cell lines (e.g., Chang cells), this entry process involves a signaling pathway requiring stimulation of the phosphatidylcholine specific phospholipase and acidic sphingomyelinase which results in the generation of the second messagers diacylglycerol and ceramide, respectively [  8.	transcription
72370	1	336235	7	NULL	NULL	0	NULL	SM synthase	GP		catalyzes					SM biosynthesis	Process	main pathway of			NULL	mammalian cells	0	NULL	NULL	NULL	gw60_jbiolchem_276_16_12797_s_199	11278937	Since the main pathway of SM biosynthesis in mammalian cells is catalyzed by SM synthase, and this occurs primarily through the transfer of the phosphorylcholine group from phosphatidylcholine to ceramide, the reaction products are both SM and diacylglycerol ( 38,  45,  47,  64).	transcription
72371	2	336235	7	NULL	NULL	0	NULL	phosphatidylcholine	Chemical	  phosphorylcholine group	transferred to					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_16_12797_s_199	11278937	Since the main pathway of SM biosynthesis in mammalian cells is catalyzed by SM synthase, and this occurs primarily through the transfer of the phosphorylcholine group from phosphatidylcholine to ceramide, the reaction products are both SM and diacylglycerol ( 38,  45,  47,  64).	transcription
72372	3	336235	7	NULL	NULL	0	NULL	statement 1	Process		occur through					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_16_12797_s_199	11278937	Since the main pathway of SM biosynthesis in mammalian cells is catalyzed by SM synthase, and this occurs primarily through the transfer of the phosphorylcholine group from phosphatidylcholine to ceramide, the reaction products are both SM and diacylglycerol ( 38,  45,  47,  64).	transcription
72373	4	336235	7	NULL	NULL	0	NULL	SM	Chemical		reaction product of					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_16_12797_s_199	11278937	Since the main pathway of SM biosynthesis in mammalian cells is catalyzed by SM synthase, and this occurs primarily through the transfer of the phosphorylcholine group from phosphatidylcholine to ceramide, the reaction products are both SM and diacylglycerol ( 38,  45,  47,  64).	transcription
72374	5	336235	7	NULL	NULL	0	NULL	diacylglycerol	Chemical		reaction product of					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_16_12797_s_199	11278937	Since the main pathway of SM biosynthesis in mammalian cells is catalyzed by SM synthase, and this occurs primarily through the transfer of the phosphorylcholine group from phosphatidylcholine to ceramide, the reaction products are both SM and diacylglycerol ( 38,  45,  47,  64).	transcription
72375	1	336236	7	NULL	NULL	0	NULL	DAG	Chemical		generated by					PC-PLC	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27730_s_24	9346915	Diacylglycerol (DAG) generated by a phosphatidylcholine-specific phospholipase C (PC-PLC) has been reported to serve as important factor of activation of A-SMase, which, through the generation of ceramide, is a co-factor for the activation of NFkappaB ( 27).	transcription
72376	2	336236	7	NULL	NULL	0	NULL	DAG	Chemical		important factor for					A-SMase	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27730_s_24	9346915	Diacylglycerol (DAG) generated by a phosphatidylcholine-specific phospholipase C (PC-PLC) has been reported to serve as important factor of activation of A-SMase, which, through the generation of ceramide, is a co-factor for the activation of NFkappaB ( 27).	transcription
72377	3	336236	7	NULL	NULL	0	NULL	 A-SMase	GP		generates					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27730_s_24	9346915	Diacylglycerol (DAG) generated by a phosphatidylcholine-specific phospholipase C (PC-PLC) has been reported to serve as important factor of activation of A-SMase, which, through the generation of ceramide, is a co-factor for the activation of NFkappaB ( 27).	transcription
72378	4	336236	7	NULL	NULL	0	NULL	ceramide	Chemical		cofactor for					NFkappaB	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27730_s_24	9346915	Diacylglycerol (DAG) generated by a phosphatidylcholine-specific phospholipase C (PC-PLC) has been reported to serve as important factor of activation of A-SMase, which, through the generation of ceramide, is a co-factor for the activation of NFkappaB ( 27).	transcription
72379	5	336236	7	NULL	NULL	0	NULL	DAG	Chemical		is					Diacylglycerol	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27730_s_24	9346915	Diacylglycerol (DAG) generated by a phosphatidylcholine-specific phospholipase C (PC-PLC) has been reported to serve as important factor of activation of A-SMase, which, through the generation of ceramide, is a co-factor for the activation of NFkappaB ( 27).	transcription
72380	6	336236	7	NULL	NULL	0	NULL	PC-PLC	GP		is					phosphatidylcholine-specific phospholipase C	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_44_27730_s_24	9346915	Diacylglycerol (DAG) generated by a phosphatidylcholine-specific phospholipase C (PC-PLC) has been reported to serve as important factor of activation of A-SMase, which, through the generation of ceramide, is a co-factor for the activation of NFkappaB ( 27).	transcription
72492	1	336237	7	NULL	NULL	0	NULL	TNF	GP		activates 					NF-kappaB	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_12_6607_s_18	9506955	For example, the phosphatidylcholine-specific phospholipase C (PC-PLC) as part of the sphingomyelin pathway upstream of the second messenger ceramide has been implicated in TNF activation of NF-kappaB ( 14).	transcription
72493	2	336237	7	NULL	NULL	0	NULL	PC-PLC	GP		implicated in					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_12_6607_s_18	9506955	For example, the phosphatidylcholine-specific phospholipase C (PC-PLC) as part of the sphingomyelin pathway upstream of the second messenger ceramide has been implicated in TNF activation of NF-kappaB ( 14).	transcription
72503	3	336237	7	NULL	NULL	0	NULL	PC-PLC	GP		is part of					sphingomyelin pathway	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_12_6607_s_18	9506955	For example, the phosphatidylcholine-specific phospholipase C (PC-PLC) as part of the sphingomyelin pathway upstream of the second messenger ceramide has been implicated in TNF activation of NF-kappaB ( 14).	transcription
72504	4	336237	7	NULL	NULL	0	NULL	PC-PLC	GP		upstream of					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_12_6607_s_18	9506955	For example, the phosphatidylcholine-specific phospholipase C (PC-PLC) as part of the sphingomyelin pathway upstream of the second messenger ceramide has been implicated in TNF activation of NF-kappaB ( 14).	transcription
72505	5	336237	7	NULL	NULL	0	NULL	ceramide	Chemical		is a type of					second messenger	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_12_6607_s_18	9506955	For example, the phosphatidylcholine-specific phospholipase C (PC-PLC) as part of the sphingomyelin pathway upstream of the second messenger ceramide has been implicated in TNF activation of NF-kappaB ( 14).	transcription
72506	6	336237	7	NULL	NULL	0	NULL	PC-PLC	GP		is					phosphatidylcholine-specific phospholipase C	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_12_6607_s_18	9506955	For example, the phosphatidylcholine-specific phospholipase C (PC-PLC) as part of the sphingomyelin pathway upstream of the second messenger ceramide has been implicated in TNF activation of NF-kappaB ( 14).	transcription
72507	1	336238	7	NULL	NULL	NULL	NULL	mAb90 	GP	mouse	bind					HLA class I	GP	human	alpha 1 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_9_5060_s_4	9478956	The mouse mAb90 or the rat YTH862 monoclonal antibodies which bind the human HLA class I alpha1 domain induced the production of ceramide which was blocked by addition of the phosphatidylcholine-dependent phospholipase C inhibitor, D609.	transcription
72508	2	336238	7	NULL	NULL	NULL	NULL	YTH862	GP	rat	bind					HLA class I	Gp	human	alpha 1 domain		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_9_5060_s_4	9478956	The mouse mAb90 or the rat YTH862 monoclonal antibodies which bind the human HLA class I alpha1 domain induced the production of ceramide which was blocked by addition of the phosphatidylcholine-dependent phospholipase C inhibitor, D609.	transcription
72509	4	336238	7	NULL	NULL	NULL	NULL	statement 3	Process		induce					ceramide	Chemical	production of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_273_9_5060_s_4	9478956	The mouse mAb90 or the rat YTH862 monoclonal antibodies which bind the human HLA class I alpha1 domain induced the production of ceramide which was blocked by addition of the phosphatidylcholine-dependent phospholipase C inhibitor, D609.	transcription
72510	3	336238	7	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_5060_s_4	9478956	The mouse mAb90 or the rat YTH862 monoclonal antibodies which bind the human HLA class I alpha1 domain induced the production of ceramide which was blocked by addition of the phosphatidylcholine-dependent phospholipase C inhibitor, D609.	transcription
72511	5	336238	7	NULL	NULL	0	NULL	D609	Chemical		block					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_5060_s_4	9478956	The mouse mAb90 or the rat YTH862 monoclonal antibodies which bind the human HLA class I alpha1 domain induced the production of ceramide which was blocked by addition of the phosphatidylcholine-dependent phospholipase C inhibitor, D609.	transcription
72512	6	336238	7	NULL	NULL	0	NULL	D609	Chemical		is a inhibitor of					phosphatidylcholine-dependent phospholipase C	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_5060_s_4	9478956	The mouse mAb90 or the rat YTH862 monoclonal antibodies which bind the human HLA class I alpha1 domain induced the production of ceramide which was blocked by addition of the phosphatidylcholine-dependent phospholipase C inhibitor, D609.	transcription
72513	7	336238	7	NULL	NULL	0	NULL	 mAb90	GP	mouse	is a type of					monoclonal antibody	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_5060_s_4	9478956	The mouse mAb90 or the rat YTH862 monoclonal antibodies which bind the human HLA class I alpha1 domain induced the production of ceramide which was blocked by addition of the phosphatidylcholine-dependent phospholipase C inhibitor, D609.	transcription
72514	8	336238	7	NULL	NULL	0	NULL	YTH862	GP	rat	is a type of					monoclonal antibody	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_273_9_5060_s_4	9478956	The mouse mAb90 or the rat YTH862 monoclonal antibodies which bind the human HLA class I alpha1 domain induced the production of ceramide which was blocked by addition of the phosphatidylcholine-dependent phospholipase C inhibitor, D609.	transcription
72515	1	336239	7	NULL	NULL	0	NULL	rCTB	GP		inhibit					sphingomyelin	Chemical	synthesis of			NULL		0	NULL	NULL	NULL	abs-batch0530-0539_j-immunol_175_9_16237053_s_5	16237053	First, rCTB inhibits sphingomyelin synthesis;  second, it enhances phosphatidylcholine synthesis; and third, it activates  a raft-resident neutral sphingomyelinase resembling to neutral sphingomyelinase  type 1, thus generating a transient ceramide production.	transcription
72516	2	336239	7	NULL	NULL	0	NULL	rCTB	GP		enhance					phosphatidylcholine	Chemical	synthesis of			NULL		0	NULL	NULL	NULL	abs-batch0530-0539_j-immunol_175_9_16237053_s_5	16237053	First, rCTB inhibits sphingomyelin synthesis;  second, it enhances phosphatidylcholine synthesis; and third, it activates  a raft-resident neutral sphingomyelinase resembling to neutral sphingomyelinase  type 1, thus generating a transient ceramide production.	transcription
72517	3	336239	7	NULL	NULL	0	NULL	rCTB	GP		activates					sphingomyelinase	GP	raft-resident neutral 			NULL		0	NULL	NULL	NULL	abs-batch0530-0539_j-immunol_175_9_16237053_s_5	16237053	First, rCTB inhibits sphingomyelin synthesis;  second, it enhances phosphatidylcholine synthesis; and third, it activates  a raft-resident neutral sphingomyelinase resembling to neutral sphingomyelinase  type 1, thus generating a transient ceramide production.	transcription
72518	4	336239	7	NULL	NULL	0	NULL	statement 3	Process		generate					ceramide	Chemical	transient production of			NULL		0	NULL	NULL	NULL	abs-batch0530-0539_j-immunol_175_9_16237053_s_5	16237053	First, rCTB inhibits sphingomyelin synthesis;  second, it enhances phosphatidylcholine synthesis; and third, it activates  a raft-resident neutral sphingomyelinase resembling to neutral sphingomyelinase  type 1, thus generating a transient ceramide production.	transcription
72519	5	336239	7	NULL	NULL	0	NULL	sphingomyelinase	GP	raft-resident neutral	resemble					sphingomyelinase	GP	neutral			NULL		0	NULL	NULL	NULL	abs-batch0530-0539_j-immunol_175_9_16237053_s_5	16237053	First, rCTB inhibits sphingomyelin synthesis;  second, it enhances phosphatidylcholine synthesis; and third, it activates  a raft-resident neutral sphingomyelinase resembling to neutral sphingomyelinase  type 1, thus generating a transient ceramide production.	transcription
72520	1	336240	7	NULL	NULL	0	NULL	ceramide	Chemical		activates					intracellular pathways	Process				NULL		0	NULL	NULL	NULL	gw70_circulation_107_10_1418_s_134	12642364	Role of Sphingomyelin-Ceramide Signaling Pathway in TNF-alpha - induced Effects   To explore the potential involvement of the ceramide-activated intracellular pathways in TNF-alpha - induced ROS production and mtDNA damage, we used D609, an inhibitor of the phosphatidylcholine-specific phospholipase C pathway and hence an indirect inhibitor of acid sphingomyelinase.	transcription
72521	2	336240	7	NULL	NULL	0	NULL	TNF-alpha	GP		induce					ROS	Chemical	production of			NULL		0	NULL	NULL	NULL	gw70_circulation_107_10_1418_s_134	12642364	Role of Sphingomyelin-Ceramide Signaling Pathway in TNF-alpha - induced Effects   To explore the potential involvement of the ceramide-activated intracellular pathways in TNF-alpha - induced ROS production and mtDNA damage, we used D609, an inhibitor of the phosphatidylcholine-specific phospholipase C pathway and hence an indirect inhibitor of acid sphingomyelinase.	transcription
72522	3	336240	7	NULL	NULL	0	NULL	TNF-alpha	GP		induce					mtDNA	NucleicAcid	damage of			NULL		0	NULL	NULL	NULL	gw70_circulation_107_10_1418_s_134	12642364	Role of Sphingomyelin-Ceramide Signaling Pathway in TNF-alpha - induced Effects   To explore the potential involvement of the ceramide-activated intracellular pathways in TNF-alpha - induced ROS production and mtDNA damage, we used D609, an inhibitor of the phosphatidylcholine-specific phospholipase C pathway and hence an indirect inhibitor of acid sphingomyelinase.	transcription
72523	4	336240	7	NULL	NULL	0	NULL	D609	Chemical		is a inhibitor of					phosphatidylcholine-specific phospholipase C pathway 	Process				NULL		0	NULL	NULL	NULL	gw70_circulation_107_10_1418_s_134	12642364	Role of Sphingomyelin-Ceramide Signaling Pathway in TNF-alpha - induced Effects   To explore the potential involvement of the ceramide-activated intracellular pathways in TNF-alpha - induced ROS production and mtDNA damage, we used D609, an inhibitor of the phosphatidylcholine-specific phospholipase C pathway and hence an indirect inhibitor of acid sphingomyelinase.	transcription
72524	5	336240	7	NULL	NULL	0	NULL	D609	Chemical		inhibitor of		indirect			acid sphingomyelinase	GP				NULL		0	NULL	NULL	NULL	gw70_circulation_107_10_1418_s_134	12642364	Role of Sphingomyelin-Ceramide Signaling Pathway in TNF-alpha - induced Effects   To explore the potential involvement of the ceramide-activated intracellular pathways in TNF-alpha - induced ROS production and mtDNA damage, we used D609, an inhibitor of the phosphatidylcholine-specific phospholipase C pathway and hence an indirect inhibitor of acid sphingomyelinase.	transcription
72525	1	336241	7	NULL	NULL	0	NULL	HS	PhysicalPhenomenon		induce					ceramide	Chemical	generation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_11_7668_s_262	10713077	These results strongly suggested the involvement of sphingomyelinase activation in HS-induced ceramide generation, even though it is unable to eliminate completely the role of other enzymes including phospholipase D type of sphingomyelinase and ceramide:phosphatidylcholine phosphocholine transferase in HS-induced apoptosis.	transcription
72526	2	336241	7	NULL	NULL	0	NULL	sphingomyelinase	GP	activation of	occur in					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_11_7668_s_262	10713077	These results strongly suggested the involvement of sphingomyelinase activation in HS-induced ceramide generation, even though it is unable to eliminate completely the role of other enzymes including phospholipase D type of sphingomyelinase and ceramide:phosphatidylcholine phosphocholine transferase in HS-induced apoptosis.	transcription
72527	3	336241	7	NULL	NULL	0	NULL	HS	PhysicalPhenomenon		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_11_7668_s_262	10713077	These results strongly suggested the involvement of sphingomyelinase activation in HS-induced ceramide generation, even though it is unable to eliminate completely the role of other enzymes including phospholipase D type of sphingomyelinase and ceramide:phosphatidylcholine phosphocholine transferase in HS-induced apoptosis.	transcription
72528	4	336241	7	NULL	NULL	0	NULL	phospholipase D type of sphingomyelinase	GP		is involved in					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_11_7668_s_262	10713077	These results strongly suggested the involvement of sphingomyelinase activation in HS-induced ceramide generation, even though it is unable to eliminate completely the role of other enzymes including phospholipase D type of sphingomyelinase and ceramide:phosphatidylcholine phosphocholine transferase in HS-induced apoptosis.	transcription
72529	5	336241	7	NULL	NULL	0	NULL	ceramide:phosphatidylcholine phosphocholine transferase	GP		is involved in					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_11_7668_s_262	10713077	These results strongly suggested the involvement of sphingomyelinase activation in HS-induced ceramide generation, even though it is unable to eliminate completely the role of other enzymes including phospholipase D type of sphingomyelinase and ceramide:phosphatidylcholine phosphocholine transferase in HS-induced apoptosis.	transcription
72530	1	336242	7	NULL	NULL	0	NULL	Choline	Chemical	deficiency of	induce					apoptosis	Process				NULL	pc12 cells 	0	NULL	NULL	NULL	gw70_brainresmolbrainres_134_2_309_s_513	15836926	[75] C.L. Yen, M.H. Mar and S.H. Zeisel, Choline deficiency-induced apoptosis in pc12  cells is associated with diminished membrane phosphatidylcholine and sphingomyelin,  accumulation of ceramide and diacylglycerol, and activation of a caspase,  FASEB J. 13 (1999), pp. 135-142.	transcription
72531	2	336242	7	NULL	NULL	0	NULL	statement 1	Process		associated with					 phosphatidylcholine	Chemical	diminished;; membrane			NULL		0	NULL	NULL	NULL	gw70_brainresmolbrainres_134_2_309_s_513	15836926	[75] C.L. Yen, M.H. Mar and S.H. Zeisel, Choline deficiency-induced apoptosis in pc12  cells is associated with diminished membrane phosphatidylcholine and sphingomyelin,  accumulation of ceramide and diacylglycerol, and activation of a caspase,  FASEB J. 13 (1999), pp. 135-142.	transcription
72532	3	336242	7	NULL	NULL	0	NULL	statement 1	Process		associated with					sphingomyelin	Chemical	diminished;; membrane			NULL		0	NULL	NULL	NULL	gw70_brainresmolbrainres_134_2_309_s_513	15836926	[75] C.L. Yen, M.H. Mar and S.H. Zeisel, Choline deficiency-induced apoptosis in pc12  cells is associated with diminished membrane phosphatidylcholine and sphingomyelin,  accumulation of ceramide and diacylglycerol, and activation of a caspase,  FASEB J. 13 (1999), pp. 135-142.	transcription
72533	4	336242	7	NULL	NULL	0	NULL	statement 1	Process		associated with					ceramide	Chemical	accumulation of			NULL		0	NULL	NULL	NULL	gw70_brainresmolbrainres_134_2_309_s_513	15836926	[75] C.L. Yen, M.H. Mar and S.H. Zeisel, Choline deficiency-induced apoptosis in pc12  cells is associated with diminished membrane phosphatidylcholine and sphingomyelin,  accumulation of ceramide and diacylglycerol, and activation of a caspase,  FASEB J. 13 (1999), pp. 135-142.	transcription
72534	5	336242	7	NULL	NULL	0	NULL	statement 1	Process		associated with					diacylglycerol	Chemical	accumulation of			NULL		0	NULL	NULL	NULL	gw70_brainresmolbrainres_134_2_309_s_513	15836926	[75] C.L. Yen, M.H. Mar and S.H. Zeisel, Choline deficiency-induced apoptosis in pc12  cells is associated with diminished membrane phosphatidylcholine and sphingomyelin,  accumulation of ceramide and diacylglycerol, and activation of a caspase,  FASEB J. 13 (1999), pp. 135-142.	transcription
72535	6	336242	7	NULL	NULL	0	NULL	statement 1	Process		associated with					caspase	GP	activation of			NULL		0	NULL	NULL	NULL	gw70_brainresmolbrainres_134_2_309_s_513	15836926	[75] C.L. Yen, M.H. Mar and S.H. Zeisel, Choline deficiency-induced apoptosis in pc12  cells is associated with diminished membrane phosphatidylcholine and sphingomyelin,  accumulation of ceramide and diacylglycerol, and activation of a caspase,  FASEB J. 13 (1999), pp. 135-142.	transcription
72536	1	336243	7	NULL	NULL	0	NULL	CD1b 	GP		bind		strongly			phosphatidylcholine	Chemical	NBD-labeled			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_1_299_s_6	14551186	Whereas group 1 CD1 isoforms (CD1b and CD1c) show stronger binding of nitrobenzoxadiazole (NBD)-labeled dialkyl-based ligands (phosphatidylcholine, sphingomyelin, and ceramide), group 2 CD1 (CD1d) proteins were stronger binders of small hydrophobic probes such as 1-anilinonaphthalene-8-sulfonic acid and 4,4''-dianilino-1,1''-naphthyl-5,5''-disulfonic acid.	transcription
72537	2	336243	7	NULL	NULL	NULL	NULL	CD1b	GP		bind		strongly			sphingomyelin	Chemical	NBD-labeled			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_1_299_s_6	14551186	Whereas group 1 CD1 isoforms (CD1b and CD1c) show stronger binding of nitrobenzoxadiazole (NBD)-labeled dialkyl-based ligands (phosphatidylcholine, sphingomyelin, and ceramide), group 2 CD1 (CD1d) proteins were stronger binders of small hydrophobic probes such as 1-anilinonaphthalene-8-sulfonic acid and 4,4''-dianilino-1,1''-naphthyl-5,5''-disulfonic acid.	transcription
72538	3	336243	7	NULL	NULL	0	NULL	CD1b	GP		bind		strongly			ceramide	Chemical	NBD-labeled			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_1_299_s_6	14551186	Whereas group 1 CD1 isoforms (CD1b and CD1c) show stronger binding of nitrobenzoxadiazole (NBD)-labeled dialkyl-based ligands (phosphatidylcholine, sphingomyelin, and ceramide), group 2 CD1 (CD1d) proteins were stronger binders of small hydrophobic probes such as 1-anilinonaphthalene-8-sulfonic acid and 4,4''-dianilino-1,1''-naphthyl-5,5''-disulfonic acid.	transcription
72539	4	336243	7	NULL	NULL	0	NULL	NBD	Chemical		is					nitrobenzoxadiazole	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_1_299_s_6	14551186	Whereas group 1 CD1 isoforms (CD1b and CD1c) show stronger binding of nitrobenzoxadiazole (NBD)-labeled dialkyl-based ligands (phosphatidylcholine, sphingomyelin, and ceramide), group 2 CD1 (CD1d) proteins were stronger binders of small hydrophobic probes such as 1-anilinonaphthalene-8-sulfonic acid and 4,4''-dianilino-1,1''-naphthyl-5,5''-disulfonic acid.	transcription
72540	5	336243	7	NULL	NULL	0	NULL	CD1c	GP		bind		strongly			phosphatidylcholine	Chemical	NBD-labeled			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_1_299_s_6	14551186	Whereas group 1 CD1 isoforms (CD1b and CD1c) show stronger binding of nitrobenzoxadiazole (NBD)-labeled dialkyl-based ligands (phosphatidylcholine, sphingomyelin, and ceramide), group 2 CD1 (CD1d) proteins were stronger binders of small hydrophobic probes such as 1-anilinonaphthalene-8-sulfonic acid and 4,4''-dianilino-1,1''-naphthyl-5,5''-disulfonic acid.	transcription
72541	6	336243	7	NULL	NULL	0	NULL	CD1c	GP		bind		strongly			sphingomyelin	Chemical	NBD-labeled			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_1_299_s_6	14551186	Whereas group 1 CD1 isoforms (CD1b and CD1c) show stronger binding of nitrobenzoxadiazole (NBD)-labeled dialkyl-based ligands (phosphatidylcholine, sphingomyelin, and ceramide), group 2 CD1 (CD1d) proteins were stronger binders of small hydrophobic probes such as 1-anilinonaphthalene-8-sulfonic acid and 4,4''-dianilino-1,1''-naphthyl-5,5''-disulfonic acid.	transcription
72542	7	336243	7	NULL	NULL	0	NULL	CD1c	GP		bind		strongly			ceramide	Chemical	NBD-labeled			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_1_299_s_6	14551186	Whereas group 1 CD1 isoforms (CD1b and CD1c) show stronger binding of nitrobenzoxadiazole (NBD)-labeled dialkyl-based ligands (phosphatidylcholine, sphingomyelin, and ceramide), group 2 CD1 (CD1d) proteins were stronger binders of small hydrophobic probes such as 1-anilinonaphthalene-8-sulfonic acid and 4,4''-dianilino-1,1''-naphthyl-5,5''-disulfonic acid.	transcription
72543	8	336243	7	NULL	NULL	0	NULL	CD1d	GP		bind		strongly			1-anilinonaphthalene-8-sulfonic acid	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_1_299_s_6	14551186	Whereas group 1 CD1 isoforms (CD1b and CD1c) show stronger binding of nitrobenzoxadiazole (NBD)-labeled dialkyl-based ligands (phosphatidylcholine, sphingomyelin, and ceramide), group 2 CD1 (CD1d) proteins were stronger binders of small hydrophobic probes such as 1-anilinonaphthalene-8-sulfonic acid and 4,4''-dianilino-1,1''-naphthyl-5,5''-disulfonic acid.	transcription
72544	9	336243	7	NULL	NULL	0	NULL	CD1d	GP		bind		strongly			4,4''-dianilino-1,1''-naphthyl-5,5''-disulfonic acid	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_1_299_s_6	14551186	Whereas group 1 CD1 isoforms (CD1b and CD1c) show stronger binding of nitrobenzoxadiazole (NBD)-labeled dialkyl-based ligands (phosphatidylcholine, sphingomyelin, and ceramide), group 2 CD1 (CD1d) proteins were stronger binders of small hydrophobic probes such as 1-anilinonaphthalene-8-sulfonic acid and 4,4''-dianilino-1,1''-naphthyl-5,5''-disulfonic acid.	transcription
72545	10	336243	7	NULL	NULL	0	NULL	phosphatidylcholine	Chemical		is a type of					dialkyl-based ligands 	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_1_299_s_6	14551186	Whereas group 1 CD1 isoforms (CD1b and CD1c) show stronger binding of nitrobenzoxadiazole (NBD)-labeled dialkyl-based ligands (phosphatidylcholine, sphingomyelin, and ceramide), group 2 CD1 (CD1d) proteins were stronger binders of small hydrophobic probes such as 1-anilinonaphthalene-8-sulfonic acid and 4,4''-dianilino-1,1''-naphthyl-5,5''-disulfonic acid.	transcription
72546	11	336243	7	NULL	NULL	0	NULL	sphingomyelin	Chemical		is a type of					dialkyl-based ligands 	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_1_299_s_6	14551186	Whereas group 1 CD1 isoforms (CD1b and CD1c) show stronger binding of nitrobenzoxadiazole (NBD)-labeled dialkyl-based ligands (phosphatidylcholine, sphingomyelin, and ceramide), group 2 CD1 (CD1d) proteins were stronger binders of small hydrophobic probes such as 1-anilinonaphthalene-8-sulfonic acid and 4,4''-dianilino-1,1''-naphthyl-5,5''-disulfonic acid.	transcription
72547	12	336243	7	NULL	NULL	0	NULL	ceramide	Chemical		is a type of					dialkyl-based ligands 	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_1_299_s_6	14551186	Whereas group 1 CD1 isoforms (CD1b and CD1c) show stronger binding of nitrobenzoxadiazole (NBD)-labeled dialkyl-based ligands (phosphatidylcholine, sphingomyelin, and ceramide), group 2 CD1 (CD1d) proteins were stronger binders of small hydrophobic probes such as 1-anilinonaphthalene-8-sulfonic acid and 4,4''-dianilino-1,1''-naphthyl-5,5''-disulfonic acid.	transcription
72548	13	336243	7	NULL	NULL	0	NULL	1-anilinonaphthalene-8-sulfonic acid 	Chemical		is a type of					small hydrophobic probes	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_1_299_s_6	14551186	Whereas group 1 CD1 isoforms (CD1b and CD1c) show stronger binding of nitrobenzoxadiazole (NBD)-labeled dialkyl-based ligands (phosphatidylcholine, sphingomyelin, and ceramide), group 2 CD1 (CD1d) proteins were stronger binders of small hydrophobic probes such as 1-anilinonaphthalene-8-sulfonic acid and 4,4''-dianilino-1,1''-naphthyl-5,5''-disulfonic acid.	transcription
72549	14	336243	7	NULL	NULL	0	NULL	4,4''-dianilino-1,1''-naphthyl-5,5''-disulfonic acid	Chemical		is a type of					small hydrophobic probes	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_1_299_s_6	14551186	Whereas group 1 CD1 isoforms (CD1b and CD1c) show stronger binding of nitrobenzoxadiazole (NBD)-labeled dialkyl-based ligands (phosphatidylcholine, sphingomyelin, and ceramide), group 2 CD1 (CD1d) proteins were stronger binders of small hydrophobic probes such as 1-anilinonaphthalene-8-sulfonic acid and 4,4''-dianilino-1,1''-naphthyl-5,5''-disulfonic acid.	transcription
72550	15	336243	7	NULL	NULL	0	NULL	CD1b	GP		is a type of					CD1 isoform	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_1_299_s_6	14551186	Whereas group 1 CD1 isoforms (CD1b and CD1c) show stronger binding of nitrobenzoxadiazole (NBD)-labeled dialkyl-based ligands (phosphatidylcholine, sphingomyelin, and ceramide), group 2 CD1 (CD1d) proteins were stronger binders of small hydrophobic probes such as 1-anilinonaphthalene-8-sulfonic acid and 4,4''-dianilino-1,1''-naphthyl-5,5''-disulfonic acid.	transcription
72551	16	336243	7	NULL	NULL	0	NULL	CD1c	GP		is a type of					CD1 isoform	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_1_299_s_6	14551186	Whereas group 1 CD1 isoforms (CD1b and CD1c) show stronger binding of nitrobenzoxadiazole (NBD)-labeled dialkyl-based ligands (phosphatidylcholine, sphingomyelin, and ceramide), group 2 CD1 (CD1d) proteins were stronger binders of small hydrophobic probes such as 1-anilinonaphthalene-8-sulfonic acid and 4,4''-dianilino-1,1''-naphthyl-5,5''-disulfonic acid.	transcription
72552	1	336244	7	NULL	NULL	0	NULL	ceramide	Chemical	generation of	derived from					sphingomyelin	Chemical				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_55_1_118_s_3	9882705	The present study demonstrates that clinically relevant concentrations of the chemotherapeutic drugs daunorubicin and mitoxantrone (0.2-1 muM) transiently stimulated concurrently with sphingomyelin-derived ceramide generation and diacylglycerol and phosphorylcholine production within 4 to 10 min via phospholipase C hydrolysis of phosphatidylcholine.	transcription
72553	2	336244	7	NULL	NULL	NULL	NULL	daunorubicin	Chemical		stimulate		transiently			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_55_1_118_s_3	9882705	The present study demonstrates that clinically relevant concentrations of the chemotherapeutic drugs daunorubicin and mitoxantrone (0.2-1 muM) transiently stimulated concurrently with sphingomyelin-derived ceramide generation and diacylglycerol and phosphorylcholine production within 4 to 10 min via phospholipase C hydrolysis of phosphatidylcholine.	transcription
72554	3	336244	7	NULL	NULL	0	NULL	mitoxantrone	Chemical		stimulate		transiently			statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_55_1_118_s_3	9882705	The present study demonstrates that clinically relevant concentrations of the chemotherapeutic drugs daunorubicin and mitoxantrone (0.2-1 muM) transiently stimulated concurrently with sphingomyelin-derived ceramide generation and diacylglycerol and phosphorylcholine production within 4 to 10 min via phospholipase C hydrolysis of phosphatidylcholine.	transcription
72555	4	336244	7	NULL	NULL	0	NULL	daunorubicin	Chemical		stimulate		transiently			diacylglycerol	Chemical	production of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_55_1_118_s_3	9882705	The present study demonstrates that clinically relevant concentrations of the chemotherapeutic drugs daunorubicin and mitoxantrone (0.2-1 muM) transiently stimulated concurrently with sphingomyelin-derived ceramide generation and diacylglycerol and phosphorylcholine production within 4 to 10 min via phospholipase C hydrolysis of phosphatidylcholine.	transcription
72556	5	336244	7	NULL	NULL	NULL	NULL	mitoxantrone	Chemical		stimulate		transiently			diacylglycerol	Chemical	production of			NULL		NULL	NULL	NULL	NULL	gw60_molpharmacol_55_1_118_s_3	9882705	The present study demonstrates that clinically relevant concentrations of the chemotherapeutic drugs daunorubicin and mitoxantrone (0.2-1 muM) transiently stimulated concurrently with sphingomyelin-derived ceramide generation and diacylglycerol and phosphorylcholine production within 4 to 10 min via phospholipase C hydrolysis of phosphatidylcholine.	transcription
72557	6	336244	7	NULL	NULL	0	NULL	daunorubicin	Chemical		stimulate		transiently			phosphoryl choline	Chemical	production of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_55_1_118_s_3	9882705	The present study demonstrates that clinically relevant concentrations of the chemotherapeutic drugs daunorubicin and mitoxantrone (0.2-1 muM) transiently stimulated concurrently with sphingomyelin-derived ceramide generation and diacylglycerol and phosphorylcholine production within 4 to 10 min via phospholipase C hydrolysis of phosphatidylcholine.	transcription
72558	7	336244	7	NULL	NULL	0	NULL	mitoxantrone	Chemical		stimulate		transiently			phosphoryl choline	Chemical	production of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_55_1_118_s_3	9882705	The present study demonstrates that clinically relevant concentrations of the chemotherapeutic drugs daunorubicin and mitoxantrone (0.2-1 muM) transiently stimulated concurrently with sphingomyelin-derived ceramide generation and diacylglycerol and phosphorylcholine production within 4 to 10 min via phospholipase C hydrolysis of phosphatidylcholine.	transcription
72559	8	336244	7	NULL	NULL	0	NULL	 phospholipase C 	GP		hydrolyze					phosphatidylcholine	Chemical				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_55_1_118_s_3	9882705	The present study demonstrates that clinically relevant concentrations of the chemotherapeutic drugs daunorubicin and mitoxantrone (0.2-1 muM) transiently stimulated concurrently with sphingomyelin-derived ceramide generation and diacylglycerol and phosphorylcholine production within 4 to 10 min via phospholipase C hydrolysis of phosphatidylcholine.	transcription
72560	9	336244	7	NULL	NULL	0	NULL	phosphoryl choline	Chemical	production of	occur via					statement 8	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_55_1_118_s_3	9882705	The present study demonstrates that clinically relevant concentrations of the chemotherapeutic drugs daunorubicin and mitoxantrone (0.2-1 muM) transiently stimulated concurrently with sphingomyelin-derived ceramide generation and diacylglycerol and phosphorylcholine production within 4 to 10 min via phospholipase C hydrolysis of phosphatidylcholine.	transcription
72561	10	336244	7	NULL	NULL	0	NULL	daunorubicin 	Chemical		is a type of					chemotherapeutic drug	Chemical				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_55_1_118_s_3	9882705	The present study demonstrates that clinically relevant concentrations of the chemotherapeutic drugs daunorubicin and mitoxantrone (0.2-1 muM) transiently stimulated concurrently with sphingomyelin-derived ceramide generation and diacylglycerol and phosphorylcholine production within 4 to 10 min via phospholipase C hydrolysis of phosphatidylcholine.	transcription
72562	11	336244	7	NULL	NULL	0	NULL	mitoxantrone	Chemical		is a type of					chemotherapeutic drug	Chemical				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_55_1_118_s_3	9882705	The present study demonstrates that clinically relevant concentrations of the chemotherapeutic drugs daunorubicin and mitoxantrone (0.2-1 muM) transiently stimulated concurrently with sphingomyelin-derived ceramide generation and diacylglycerol and phosphorylcholine production within 4 to 10 min via phospholipase C hydrolysis of phosphatidylcholine.	transcription
72563	1	336245	7	NULL	NULL	0	NULL	TNF-alpha	GP		induce					transduction pathway	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_32_30527_s_37	11390371	The TNF-alpha-induced transduction pathway leading to activation of NF-kappaB has also been proposed to involve phosphatidylcholine-specific phospholipase C ( 37), sphingomyelinase ( 38,  39), and protein kinase C zeta activated by ceramide ( 40).	transcription
72564	2	336245	7	NULL	NULL	0	NULL	statement 1	Process		leads to					NF-kappaB	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_32_30527_s_37	11390371	The TNF-alpha-induced transduction pathway leading to activation of NF-kappaB has also been proposed to involve phosphatidylcholine-specific phospholipase C ( 37), sphingomyelinase ( 38,  39), and protein kinase C zeta activated by ceramide ( 40).	transcription
72565	3	336245	7	NULL	NULL	0	NULL	statement 2	Process		involve					phosphatidylcholine-specific phospholipase C	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_32_30527_s_37	11390371	The TNF-alpha-induced transduction pathway leading to activation of NF-kappaB has also been proposed to involve phosphatidylcholine-specific phospholipase C ( 37), sphingomyelinase ( 38,  39), and protein kinase C zeta activated by ceramide ( 40).	transcription
72566	4	336245	7	NULL	NULL	0	NULL	statement 2	Process		involve					sphingomyelinase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_32_30527_s_37	11390371	The TNF-alpha-induced transduction pathway leading to activation of NF-kappaB has also been proposed to involve phosphatidylcholine-specific phospholipase C ( 37), sphingomyelinase ( 38,  39), and protein kinase C zeta activated by ceramide ( 40).	transcription
72567	5	336245	7	NULL	NULL	0	NULL	ceramide	Chemical		activate					protein kinase C zeta 	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_32_30527_s_37	11390371	The TNF-alpha-induced transduction pathway leading to activation of NF-kappaB has also been proposed to involve phosphatidylcholine-specific phospholipase C ( 37), sphingomyelinase ( 38,  39), and protein kinase C zeta activated by ceramide ( 40).	transcription
72568	6	336245	7	NULL	NULL	0	NULL	statement 2	Process		involve					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_32_30527_s_37	11390371	The TNF-alpha-induced transduction pathway leading to activation of NF-kappaB has also been proposed to involve phosphatidylcholine-specific phospholipase C ( 37), sphingomyelinase ( 38,  39), and protein kinase C zeta activated by ceramide ( 40).	transcription
72569	1	336246	7	NULL	NULL	NULL	NULL	enzyme systems	GP	Membrane-associated	transmit					TR55 signals	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_15_10203_s_23	10187805	Membrane-associated enzyme systems transmitting TR55 signals include plasmamembrane-bound phospholipases such as phosphatidylcholine-specific phospholipase C ( 25), which generates the lipid second messenger molecule 1,2-diacylglycerol and a N-SMase ( 9), producing ceramide by sphingomyelin hydrolysis.	transcription
72570	2	336246	7	NULL	NULL	0	NULL	statement 1	Process		include					phosphatidylcholine-specific phospholipase C	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_15_10203_s_23	10187805	Membrane-associated enzyme systems transmitting TR55 signals include plasmamembrane-bound phospholipases such as phosphatidylcholine-specific phospholipase C ( 25), which generates the lipid second messenger molecule 1,2-diacylglycerol and a N-SMase ( 9), producing ceramide by sphingomyelin hydrolysis.	transcription
72571	3	336246	7	NULL	NULL	0	NULL	phosphatidylcholine-specific phospholipase C	GP		generate					1,2-diacylglycerol 	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_15_10203_s_23	10187805	Membrane-associated enzyme systems transmitting TR55 signals include plasmamembrane-bound phospholipases such as phosphatidylcholine-specific phospholipase C ( 25), which generates the lipid second messenger molecule 1,2-diacylglycerol and a N-SMase ( 9), producing ceramide by sphingomyelin hydrolysis.	transcription
72572	4	336246	7	NULL	NULL	0	NULL	phosphatidylcholine-specific phospholipase C 	GP		generates					N-SMase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_15_10203_s_23	10187805	Membrane-associated enzyme systems transmitting TR55 signals include plasmamembrane-bound phospholipases such as phosphatidylcholine-specific phospholipase C ( 25), which generates the lipid second messenger molecule 1,2-diacylglycerol and a N-SMase ( 9), producing ceramide by sphingomyelin hydrolysis.	transcription
72573	5	336246	7	NULL	NULL	0	NULL	sphingomyelin	Chemical		hydrolyzed to					ceramide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_15_10203_s_23	10187805	Membrane-associated enzyme systems transmitting TR55 signals include plasmamembrane-bound phospholipases such as phosphatidylcholine-specific phospholipase C ( 25), which generates the lipid second messenger molecule 1,2-diacylglycerol and a N-SMase ( 9), producing ceramide by sphingomyelin hydrolysis.	transcription
72574	6	336246	7	NULL	NULL	0	NULL	 N-SMase	GP		produce					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_15_10203_s_23	10187805	Membrane-associated enzyme systems transmitting TR55 signals include plasmamembrane-bound phospholipases such as phosphatidylcholine-specific phospholipase C ( 25), which generates the lipid second messenger molecule 1,2-diacylglycerol and a N-SMase ( 9), producing ceramide by sphingomyelin hydrolysis.	transcription
72575	7	336246	7	NULL	NULL	0	NULL	 phosphatidylcholine-specific phospholipase C	GP		is a type of					plasmamembrane-bound phospholipases 	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_15_10203_s_23	10187805	Membrane-associated enzyme systems transmitting TR55 signals include plasmamembrane-bound phospholipases such as phosphatidylcholine-specific phospholipase C ( 25), which generates the lipid second messenger molecule 1,2-diacylglycerol and a N-SMase ( 9), producing ceramide by sphingomyelin hydrolysis.	transcription
72576	8	336246	7	NULL	NULL	0	NULL	1,2-diacylglycerol	Chemical		is a type of					lipid second messenger molecule	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_15_10203_s_23	10187805	Membrane-associated enzyme systems transmitting TR55 signals include plasmamembrane-bound phospholipases such as phosphatidylcholine-specific phospholipase C ( 25), which generates the lipid second messenger molecule 1,2-diacylglycerol and a N-SMase ( 9), producing ceramide by sphingomyelin hydrolysis.	transcription
72577	1	336247	7	NULL	NULL	0	NULL	PDMP	Chemical		inhibitor of					 glucosylceramide synthase	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_97_10_5480_s_98	10792026	Cells were treated with PDMP (10 muM), an inhibitor of glucosylceramide synthase that leads to increased ceramide concentrations ( 19); D609 (25 mug/ml), which inhibits acidic sphingomyelinase activity via inhibition of the phosphatidylcholine-specific phospholipase C ( 20); or fumonisin B1 (3 muM), an inhibitor of ceramide synthase and TNF-alpha-induced apoptosis ( 21).	transcription
72578	2	336247	7	NULL	NULL	0	NULL	statement 1	Process		leads to					ceramide	Chemical	increased			NULL		0	NULL	NULL	NULL	gw60_pnas_97_10_5480_s_98	10792026	Cells were treated with PDMP (10 muM), an inhibitor of glucosylceramide synthase that leads to increased ceramide concentrations ( 19); D609 (25 mug/ml), which inhibits acidic sphingomyelinase activity via inhibition of the phosphatidylcholine-specific phospholipase C ( 20); or fumonisin B1 (3 muM), an inhibitor of ceramide synthase and TNF-alpha-induced apoptosis ( 21).	transcription
72579	3	336247	7	NULL	NULL	0	NULL	statement 2	Process		inhibit					acidic sphingomyelinase	GP	activity of			NULL		0	NULL	NULL	NULL	gw60_pnas_97_10_5480_s_98	10792026	Cells were treated with PDMP (10 muM), an inhibitor of glucosylceramide synthase that leads to increased ceramide concentrations ( 19); D609 (25 mug/ml), which inhibits acidic sphingomyelinase activity via inhibition of the phosphatidylcholine-specific phospholipase C ( 20); or fumonisin B1 (3 muM), an inhibitor of ceramide synthase and TNF-alpha-induced apoptosis ( 21).	transcription
72580	4	336247	7	NULL	NULL	NULL	NULL	statement 3	Process		occur via 					phosphatidylcholine-specific phospholipase C 	GP	inhibition of			NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_10_5480_s_98	10792026	Cells were treated with PDMP (10 muM), an inhibitor of glucosylceramide synthase that leads to increased ceramide concentrations ( 19); D609 (25 mug/ml), which inhibits acidic sphingomyelinase activity via inhibition of the phosphatidylcholine-specific phospholipase C ( 20); or fumonisin B1 (3 muM), an inhibitor of ceramide synthase and TNF-alpha-induced apoptosis ( 21).	transcription
72581	5	336247	7	NULL	NULL	0	NULL	fumonisin B1	Chemical		is an inhibitor of					ceramide synthase	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_97_10_5480_s_98	10792026	Cells were treated with PDMP (10 muM), an inhibitor of glucosylceramide synthase that leads to increased ceramide concentrations ( 19); D609 (25 mug/ml), which inhibits acidic sphingomyelinase activity via inhibition of the phosphatidylcholine-specific phospholipase C ( 20); or fumonisin B1 (3 muM), an inhibitor of ceramide synthase and TNF-alpha-induced apoptosis ( 21).	transcription
72582	6	336247	7	NULL	NULL	0	NULL	TNF-alpha	GP		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_97_10_5480_s_98	10792026	Cells were treated with PDMP (10 muM), an inhibitor of glucosylceramide synthase that leads to increased ceramide concentrations ( 19); D609 (25 mug/ml), which inhibits acidic sphingomyelinase activity via inhibition of the phosphatidylcholine-specific phospholipase C ( 20); or fumonisin B1 (3 muM), an inhibitor of ceramide synthase and TNF-alpha-induced apoptosis ( 21).	transcription
72583	7	336247	7	NULL	NULL	0	NULL	fumonisin B1	Chemical		inhibitor of					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_97_10_5480_s_98	10792026	Cells were treated with PDMP (10 muM), an inhibitor of glucosylceramide synthase that leads to increased ceramide concentrations ( 19); D609 (25 mug/ml), which inhibits acidic sphingomyelinase activity via inhibition of the phosphatidylcholine-specific phospholipase C ( 20); or fumonisin B1 (3 muM), an inhibitor of ceramide synthase and TNF-alpha-induced apoptosis ( 21).	transcription
72584	8	336247	7	NULL	NULL	0	NULL	statement 3	Process		occur via					fumonisin B1	Chemical	inhibition of			NULL		0	NULL	NULL	NULL	gw60_pnas_97_10_5480_s_98	10792026	Cells were treated with PDMP (10 muM), an inhibitor of glucosylceramide synthase that leads to increased ceramide concentrations ( 19); D609 (25 mug/ml), which inhibits acidic sphingomyelinase activity via inhibition of the phosphatidylcholine-specific phospholipase C ( 20); or fumonisin B1 (3 muM), an inhibitor of ceramide synthase and TNF-alpha-induced apoptosis ( 21).	transcription
72585	9	336247	7	NULL	NULL	0	NULL	statement 4	Process		is an alternative to					statement 8	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_97_10_5480_s_98	10792026	Cells were treated with PDMP (10 muM), an inhibitor of glucosylceramide synthase that leads to increased ceramide concentrations ( 19); D609 (25 mug/ml), which inhibits acidic sphingomyelinase activity via inhibition of the phosphatidylcholine-specific phospholipase C ( 20); or fumonisin B1 (3 muM), an inhibitor of ceramide synthase and TNF-alpha-induced apoptosis ( 21).	transcription
72586	1	336248	7	NULL	NULL	0	NULL	HDL	GP		triggers					PI-PLC	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_19_16478_s_13	12637559	HDL triggers a variety of intracellular signaling events, including activation of phosphatidylinositol- and phosphatidylcholine-specific phospholipases C and D (PI-PLC, PC-PLC, and PC-PLD), protein kinase C (PKC), mitogen-activated protein kinase (MAPK), tyrosine kinase, and heterotrimeric G-proteins ( 6,  7) but also production of cyclic AMP (cAMP), nitric oxide (NO), and ceramide ( 4) and intracellular Ca2+ release.	transcription
72587	2	336248	7	NULL	NULL	0	NULL	HDL	GP		triggers					PC-PLC	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_19_16478_s_13	12637559	HDL triggers a variety of intracellular signaling events, including activation of phosphatidylinositol- and phosphatidylcholine-specific phospholipases C and D (PI-PLC, PC-PLC, and PC-PLD), protein kinase C (PKC), mitogen-activated protein kinase (MAPK), tyrosine kinase, and heterotrimeric G-proteins ( 6,  7) but also production of cyclic AMP (cAMP), nitric oxide (NO), and ceramide ( 4) and intracellular Ca2+ release.	transcription
72588	3	336248	7	NULL	NULL	0	NULL	HDL	GP		triggers					PC-PLD	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_19_16478_s_13	12637559	HDL triggers a variety of intracellular signaling events, including activation of phosphatidylinositol- and phosphatidylcholine-specific phospholipases C and D (PI-PLC, PC-PLC, and PC-PLD), protein kinase C (PKC), mitogen-activated protein kinase (MAPK), tyrosine kinase, and heterotrimeric G-proteins ( 6,  7) but also production of cyclic AMP (cAMP), nitric oxide (NO), and ceramide ( 4) and intracellular Ca2+ release.	transcription
72589	4	336248	7	NULL	NULL	0	NULL	HDL	GP		triggers					PKC	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_19_16478_s_13	12637559	HDL triggers a variety of intracellular signaling events, including activation of phosphatidylinositol- and phosphatidylcholine-specific phospholipases C and D (PI-PLC, PC-PLC, and PC-PLD), protein kinase C (PKC), mitogen-activated protein kinase (MAPK), tyrosine kinase, and heterotrimeric G-proteins ( 6,  7) but also production of cyclic AMP (cAMP), nitric oxide (NO), and ceramide ( 4) and intracellular Ca2+ release.	transcription
72590	5	336248	7	NULL	NULL	0	NULL	HDL	GP		triggers					MAPK	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_19_16478_s_13	12637559	HDL triggers a variety of intracellular signaling events, including activation of phosphatidylinositol- and phosphatidylcholine-specific phospholipases C and D (PI-PLC, PC-PLC, and PC-PLD), protein kinase C (PKC), mitogen-activated protein kinase (MAPK), tyrosine kinase, and heterotrimeric G-proteins ( 6,  7) but also production of cyclic AMP (cAMP), nitric oxide (NO), and ceramide ( 4) and intracellular Ca2+ release.	transcription
72591	6	336248	7	NULL	NULL	0	NULL	HDL	GP		triggers					tyrosine kinase	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_19_16478_s_13	12637559	HDL triggers a variety of intracellular signaling events, including activation of phosphatidylinositol- and phosphatidylcholine-specific phospholipases C and D (PI-PLC, PC-PLC, and PC-PLD), protein kinase C (PKC), mitogen-activated protein kinase (MAPK), tyrosine kinase, and heterotrimeric G-proteins ( 6,  7) but also production of cyclic AMP (cAMP), nitric oxide (NO), and ceramide ( 4) and intracellular Ca2+ release.	transcription
72592	7	336248	7	NULL	NULL	NULL	NULL	HDL	GP		triggers					G-proteins	GP	activation of;;heterotrimeric			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_19_16478_s_13	12637559	HDL triggers a variety of intracellular signaling events, including activation of phosphatidylinositol- and phosphatidylcholine-specific phospholipases C and D (PI-PLC, PC-PLC, and PC-PLD), protein kinase C (PKC), mitogen-activated protein kinase (MAPK), tyrosine kinase, and heterotrimeric G-proteins ( 6,  7) but also production of cyclic AMP (cAMP), nitric oxide (NO), and ceramide ( 4) and intracellular Ca2+ release.	transcription
72593	8	336248	7	NULL	NULL	0	NULL	HDL	GP		triggers					cAMP	Chemical	production of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_19_16478_s_13	12637559	HDL triggers a variety of intracellular signaling events, including activation of phosphatidylinositol- and phosphatidylcholine-specific phospholipases C and D (PI-PLC, PC-PLC, and PC-PLD), protein kinase C (PKC), mitogen-activated protein kinase (MAPK), tyrosine kinase, and heterotrimeric G-proteins ( 6,  7) but also production of cyclic AMP (cAMP), nitric oxide (NO), and ceramide ( 4) and intracellular Ca2+ release.	transcription
72594	9	336248	7	NULL	NULL	0	NULL	HDL	GP		triggers					NO	Chemical	production of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_19_16478_s_13	12637559	HDL triggers a variety of intracellular signaling events, including activation of phosphatidylinositol- and phosphatidylcholine-specific phospholipases C and D (PI-PLC, PC-PLC, and PC-PLD), protein kinase C (PKC), mitogen-activated protein kinase (MAPK), tyrosine kinase, and heterotrimeric G-proteins ( 6,  7) but also production of cyclic AMP (cAMP), nitric oxide (NO), and ceramide ( 4) and intracellular Ca2+ release.	transcription
72595	10	336248	7	NULL	NULL	0	NULL	HDL	GP		triggers					ceramide	Chemical	production of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_19_16478_s_13	12637559	HDL triggers a variety of intracellular signaling events, including activation of phosphatidylinositol- and phosphatidylcholine-specific phospholipases C and D (PI-PLC, PC-PLC, and PC-PLD), protein kinase C (PKC), mitogen-activated protein kinase (MAPK), tyrosine kinase, and heterotrimeric G-proteins ( 6,  7) but also production of cyclic AMP (cAMP), nitric oxide (NO), and ceramide ( 4) and intracellular Ca2+ release.	transcription
72596	11	336248	7	NULL	NULL	0	NULL	HDL	GP		triggers					Ca2+	Chemical	release of;;intracellular			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_19_16478_s_13	12637559	HDL triggers a variety of intracellular signaling events, including activation of phosphatidylinositol- and phosphatidylcholine-specific phospholipases C and D (PI-PLC, PC-PLC, and PC-PLD), protein kinase C (PKC), mitogen-activated protein kinase (MAPK), tyrosine kinase, and heterotrimeric G-proteins ( 6,  7) but also production of cyclic AMP (cAMP), nitric oxide (NO), and ceramide ( 4) and intracellular Ca2+ release.	transcription
72597	12	336248	7	NULL	NULL	NULL	NULL	PI-PLC	GP		is					 phosphatidylinositol-specific phospholipase C	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_19_16478_s_13	12637559	HDL triggers a variety of intracellular signaling events, including activation of phosphatidylinositol- and phosphatidylcholine-specific phospholipases C and D (PI-PLC, PC-PLC, and PC-PLD), protein kinase C (PKC), mitogen-activated protein kinase (MAPK), tyrosine kinase, and heterotrimeric G-proteins ( 6,  7) but also production of cyclic AMP (cAMP), nitric oxide (NO), and ceramide ( 4) and intracellular Ca2+ release.	transcription
72598	13	336248	7	NULL	NULL	0	NULL	PC-PLC	GP		is					phosphatidylcholine-specific phospholipase C 	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_19_16478_s_13	12637559	HDL triggers a variety of intracellular signaling events, including activation of phosphatidylinositol- and phosphatidylcholine-specific phospholipases C and D (PI-PLC, PC-PLC, and PC-PLD), protein kinase C (PKC), mitogen-activated protein kinase (MAPK), tyrosine kinase, and heterotrimeric G-proteins ( 6,  7) but also production of cyclic AMP (cAMP), nitric oxide (NO), and ceramide ( 4) and intracellular Ca2+ release.	transcription
72599	14	336248	7	NULL	NULL	NULL	NULL	PC-PLD	GP		is					phosphatidylcholine-specific phospholipase D	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_19_16478_s_13	12637559	HDL triggers a variety of intracellular signaling events, including activation of phosphatidylinositol- and phosphatidylcholine-specific phospholipases C and D (PI-PLC, PC-PLC, and PC-PLD), protein kinase C (PKC), mitogen-activated protein kinase (MAPK), tyrosine kinase, and heterotrimeric G-proteins ( 6,  7) but also production of cyclic AMP (cAMP), nitric oxide (NO), and ceramide ( 4) and intracellular Ca2+ release.	transcription
72600	15	336248	7	NULL	NULL	0	NULL	PKC	GP		is					protein kinase C	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_19_16478_s_13	12637559	HDL triggers a variety of intracellular signaling events, including activation of phosphatidylinositol- and phosphatidylcholine-specific phospholipases C and D (PI-PLC, PC-PLC, and PC-PLD), protein kinase C (PKC), mitogen-activated protein kinase (MAPK), tyrosine kinase, and heterotrimeric G-proteins ( 6,  7) but also production of cyclic AMP (cAMP), nitric oxide (NO), and ceramide ( 4) and intracellular Ca2+ release.	transcription
72601	16	336248	7	NULL	NULL	0	NULL	MAPK	GP		is					mitogen-activated protein kinase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_19_16478_s_13	12637559	HDL triggers a variety of intracellular signaling events, including activation of phosphatidylinositol- and phosphatidylcholine-specific phospholipases C and D (PI-PLC, PC-PLC, and PC-PLD), protein kinase C (PKC), mitogen-activated protein kinase (MAPK), tyrosine kinase, and heterotrimeric G-proteins ( 6,  7) but also production of cyclic AMP (cAMP), nitric oxide (NO), and ceramide ( 4) and intracellular Ca2+ release.	transcription
72602	17	336248	7	NULL	NULL	0	NULL	cAMP	Chemical		is					cyclic AMP	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_19_16478_s_13	12637559	HDL triggers a variety of intracellular signaling events, including activation of phosphatidylinositol- and phosphatidylcholine-specific phospholipases C and D (PI-PLC, PC-PLC, and PC-PLD), protein kinase C (PKC), mitogen-activated protein kinase (MAPK), tyrosine kinase, and heterotrimeric G-proteins ( 6,  7) but also production of cyclic AMP (cAMP), nitric oxide (NO), and ceramide ( 4) and intracellular Ca2+ release.	transcription
72603	18	336248	7	NULL	NULL	0	NULL	NO	Chemical		is					nitric oxide	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_19_16478_s_13	12637559	HDL triggers a variety of intracellular signaling events, including activation of phosphatidylinositol- and phosphatidylcholine-specific phospholipases C and D (PI-PLC, PC-PLC, and PC-PLD), protein kinase C (PKC), mitogen-activated protein kinase (MAPK), tyrosine kinase, and heterotrimeric G-proteins ( 6,  7) but also production of cyclic AMP (cAMP), nitric oxide (NO), and ceramide ( 4) and intracellular Ca2+ release.	transcription
72604	1	336249	7	NULL	NULL	0	NULL	p53 	GP		regulate					 p21 CIP1/WAF1	GP	transcription of			NULL		0	NULL	NULL	NULL	gw70_nature_438_7068_690_s_71	16319895	Crucially, however, the amount of p53 protein, before and after ionizing  radiation, was not dependent on APC5 and/or APC7 gene expression ( Fig. 2c, bottom), suggesting that APC5 and APC7 affect p53-regulated transcription of p21 CIP1/WAF1 directly.	transcription
72605	2	336249	7	NULL	NULL	0	NULL	APC5 	GP		affect		directly			statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_nature_438_7068_690_s_71	16319895	Crucially, however, the amount of p53 protein, before and after ionizing  radiation, was not dependent on APC5 and/or APC7 gene expression ( Fig. 2c, bottom), suggesting that APC5 and APC7 affect p53-regulated transcription of p21 CIP1/WAF1 directly.	transcription
72606	3	336249	7	NULL	NULL	0	NULL	APC7	GP		affect		directly			statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_nature_438_7068_690_s_71	16319895	Crucially, however, the amount of p53 protein, before and after ionizing  radiation, was not dependent on APC5 and/or APC7 gene expression ( Fig. 2c, bottom), suggesting that APC5 and APC7 affect p53-regulated transcription of p21 CIP1/WAF1 directly.	transcription
72607	1	336250	7	NULL	NULL	0	NULL	APC1	GP	loss of	induce					G2/M  arrest	Process				NULL		0	NULL	NULL	NULL	gw70_genesdev_18_16_1952_s_100	15314021	Loss of APC1 induces G2/M arrest and apoptosis in the absence of p53	transcription
72608	2	336250	7	NULL	NULL	0	NULL	APC1	GP	loss of	induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw70_genesdev_18_16_1952_s_100	15314021	Loss of APC1 induces G2/M arrest and apoptosis in the absence of p53	transcription
72609	3	336250	7	NULL	NULL	0	NULL	statement 2	Process		in the absence of					p53	GP				NULL		0	NULL	NULL	NULL	gw70_genesdev_18_16_1952_s_100	15314021	Loss of APC1 induces G2/M arrest and apoptosis in the absence of p53	transcription
72610	1	336251	7	NULL	NULL	0	NULL	 APC	GP		downregulates					p53	GP				NULL	TNFalpha-induced HUVECs	0	NULL	NULL	NULL	gw70_jbiolchem_280_20_19808_s_161	15769747	PAR1-dependent Down-regulation of p53 and Thrombospondin-1 by APC but Not Thrombin in TNFalpha-induced HUVECs --	transcription
72611	2	336251	7	NULL	NULL	0	NULL	APC	GP		downregulates					Thrombospondin-1	GP				NULL	TNFalpha-induced HUVECs	0	NULL	NULL	NULL	gw70_jbiolchem_280_20_19808_s_161	15769747	PAR1-dependent Down-regulation of p53 and Thrombospondin-1 by APC but Not Thrombin in TNFalpha-induced HUVECs --	transcription
72612	3	336251	7	NULL	NULL	NULL	NULL	statement 1	Process		depends on					PAR1	GP				NULL	TNFalpha-induced HUVECs	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_20_19808_s_161	15769747	PAR1-dependent Down-regulation of p53 and Thrombospondin-1 by APC but Not Thrombin in TNFalpha-induced HUVECs --	transcription
72613	4	336251	7	NULL	NULL	NULL	NULL	statement 2	Process		depends on					PAR1	GP				NULL	TNFalpha-induced HUVECs	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_20_19808_s_161	15769747	PAR1-dependent Down-regulation of p53 and Thrombospondin-1 by APC but Not Thrombin in TNFalpha-induced HUVECs --	transcription
72614	5	336251	7	NULL	NULL	NULL	NULL	APC	GP		does not downregulate					thrombin	GP				NULL	TNFalpha-induced HUVECs	NULL	NULL	NULL	NULL	gw70_jbiolchem_280_20_19808_s_161	15769747	PAR1-dependent Down-regulation of p53 and Thrombospondin-1 by APC but Not Thrombin in TNFalpha-induced HUVECs --	transcription
72615	1	336252	7	NULL	NULL	0	NULL	APC-EPCR-PAR1 	GP	signaling of	downregulates					p53 protein	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_19808_s_200	15769747	Down-regulation of p53 protein expression by APC-EPCR-PAR1 signaling.	transcription
72616	1	336253	7	NULL	NULL	0	NULL	53BP2	GP		interacts with					p53	GP				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_cancer-res_60_1_10646860_s_8	10646860	Because  53BP2 also interacts with p53 and Bcl2 and regulates p53 function, our  results suggest that APCL might be involved in the p53/Bcl2-linked pathway  of cell-cycle progression and cell death.	transcription
72617	2	336253	7	NULL	NULL	0	NULL	53BP2	GP		interacts with					Bcl2	GP				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_cancer-res_60_1_10646860_s_8	10646860	Because  53BP2 also interacts with p53 and Bcl2 and regulates p53 function, our  results suggest that APCL might be involved in the p53/Bcl2-linked pathway  of cell-cycle progression and cell death.	transcription
72618	3	336253	7	NULL	NULL	0	NULL	53BP2	GP		regulates					p53	GP	function of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_cancer-res_60_1_10646860_s_8	10646860	Because  53BP2 also interacts with p53 and Bcl2 and regulates p53 function, our  results suggest that APCL might be involved in the p53/Bcl2-linked pathway  of cell-cycle progression and cell death.	transcription
72619	4	336253	7	NULL	NULL	0	NULL	APCL	GP		be involved in		might			 cell-cycle progression	Process	p53/Bcl2-linked pathway of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_cancer-res_60_1_10646860_s_8	10646860	Because  53BP2 also interacts with p53 and Bcl2 and regulates p53 function, our  results suggest that APCL might be involved in the p53/Bcl2-linked pathway  of cell-cycle progression and cell death.	transcription
72620	5	336253	7	NULL	NULL	0	NULL	APCL	GP		be involved in		might 			cell death	Process	p53/Bcl2-linked pathway of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_cancer-res_60_1_10646860_s_8	10646860	Because  53BP2 also interacts with p53 and Bcl2 and regulates p53 function, our  results suggest that APCL might be involved in the p53/Bcl2-linked pathway  of cell-cycle progression and cell death.	transcription
72621	1	336254	7	NULL	NULL	0	NULL	DNA damage	Process		induce					APC	GP	expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_49_30619_s_87	9388195	Thus, if p53 is required for DNA damage-induced expression of  APC, then cell lines defective in wild-type functional p53 should fail to up-regulate  APC.	transcription
72622	2	336254	7	NULL	NULL	0	NULL	p53	GP		is required for					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_49_30619_s_87	9388195	Thus, if p53 is required for DNA damage-induced expression of  APC, then cell lines defective in wild-type functional p53 should fail to up-regulate  APC.	transcription
72623	3	336254	7	NULL	NULL	NULL	NULL	p53	GP	wild-type;;functional;;defective	fails to					APC	GP	up-regulate			NULL	cell lines	NULL	NULL	NULL	NULL	gw60_jbiolchem_272_49_30619_s_87	9388195	Thus, if p53 is required for DNA damage-induced expression of  APC, then cell lines defective in wild-type functional p53 should fail to up-regulate  APC.	transcription
72624	1	336255	7	NULL	NULL	0	NULL	p53 transcription factor	GP		is required for					Apc 	GP	expression of			NULL	in vitro	0	NULL	NULL	NULL	gw60_pnas_97_7_3461_s_173	10716720	The  p53 transcription factor is required for  Apc expression  in vitro ( 34), so a deficiency of  p53 may lead to silencing of  Apc expression ( 35) and enhanced adenoma formation.	transcription
72625	2	336255	7	NULL	NULL	0	NULL	p53	GP	deficiency of	leads to		may			Apc	GP	silencing of;;expression of			NULL		0	NULL	NULL	NULL	gw60_pnas_97_7_3461_s_173	10716720	The  p53 transcription factor is required for  Apc expression  in vitro ( 34), so a deficiency of  p53 may lead to silencing of  Apc expression ( 35) and enhanced adenoma formation.	transcription
72626	3	336255	7	NULL	NULL	0	NULL	p53	GP	silencing of	leads to		may			adenoma formation	Process	enhanced			NULL		0	NULL	NULL	NULL	gw60_pnas_97_7_3461_s_173	10716720	The  p53 transcription factor is required for  Apc expression  in vitro ( 34), so a deficiency of  p53 may lead to silencing of  Apc expression ( 35) and enhanced adenoma formation.	transcription
72627	1	336256	7	NULL	NULL	0	NULL	APC	GP		down-regulates					p53 transcript	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_19808_s_9	15769747	APC down-regulated transcripts for proapoptotic proteins including p53 and thrombospondin-1, but p53 was unchanged, and thrombospondin was even up-regulated by thrombin.	transcription
72628	2	336256	7	NULL	NULL	NULL	NULL	APC	GP		down-regulates					thrombospondin-1 transcript	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_20_19808_s_9	15769747	APC down-regulated transcripts for proapoptotic proteins including p53 and thrombospondin-1, but p53 was unchanged, and thrombospondin was even up-regulated by thrombin.	transcription
72629	3	336256	7	NULL	NULL	0	NULL	thrombin	GP		up-regulates					thrombospondin	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_19808_s_9	15769747	APC down-regulated transcripts for proapoptotic proteins including p53 and thrombospondin-1, but p53 was unchanged, and thrombospondin was even up-regulated by thrombin.	transcription
72630	4	336256	7	NULL	NULL	0	NULL	thrombin	GP		does not upregulate					p53	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_19808_s_9	15769747	APC down-regulated transcripts for proapoptotic proteins including p53 and thrombospondin-1, but p53 was unchanged, and thrombospondin was even up-regulated by thrombin.	transcription
72631	5	336256	7	NULL	NULL	0	NULL	p53	GP		is a type of					proapoptotic protein	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_19808_s_9	15769747	APC down-regulated transcripts for proapoptotic proteins including p53 and thrombospondin-1, but p53 was unchanged, and thrombospondin was even up-regulated by thrombin.	transcription
72632	6	336256	7	NULL	NULL	0	NULL	thrombospondin-1	GP		is a type of					proapoptotic protein	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_19808_s_9	15769747	APC down-regulated transcripts for proapoptotic proteins including p53 and thrombospondin-1, but p53 was unchanged, and thrombospondin was even up-regulated by thrombin.	transcription
72633	1	336257	7	NULL	NULL	0	NULL	doxorubicin 	Chemical		increase					p53 protein	GP	levels of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_19808_s_163	15769747	To test whether APC regulates p53, cells were treated with doxorubicin to increase p53 protein levels.	transcription
72634	1	336258	7	NULL	NULL	0	NULL	p53	GP	levels of	is limiting in					HCT-116 cells	Cell				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_49_30619_s_98	9388195	These results are consistent with the idea that p53 levels are limiting in HCT-116 cells, and the increased levels of p53 may be necessary for induced expression of APC.	transcription
72635	2	336258	7	NULL	NULL	0	NULL	p53	GP	increased levels of	is necessary for					APC	GP	induced expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_49_30619_s_98	9388195	These results are consistent with the idea that p53 levels are limiting in HCT-116 cells, and the increased levels of p53 may be necessary for induced expression of APC.	transcription
72636	1	336259	7	NULL	NULL	0	NULL	fetal-brain cDNA library	GP	human	interacts with					APCL	GP				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_cancer-res_60_1_10646860_s_4	10646860	Among 166 cDNA clones isolated from a human  fetal-brain cDNA library as candidates for interaction with APCL, 32 encoded  parts of p53-binding protein 2 (53BP2), a molecule that interacts with  p53 and Bcl2.	transcription
72637	2	336259	7	NULL	NULL	0	NULL	p53-binding protein 2	GP		interacts with			32 encoded parts of		p53	GP				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_cancer-res_60_1_10646860_s_4	10646860	Among 166 cDNA clones isolated from a human  fetal-brain cDNA library as candidates for interaction with APCL, 32 encoded  parts of p53-binding protein 2 (53BP2), a molecule that interacts with  p53 and Bcl2.	transcription
72638	3	336259	7	NULL	NULL	0	NULL	p53-binding protein 2	GP		interacts with			32 encoded parts of		Bcl2	GP				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_cancer-res_60_1_10646860_s_4	10646860	Among 166 cDNA clones isolated from a human  fetal-brain cDNA library as candidates for interaction with APCL, 32 encoded  parts of p53-binding protein 2 (53BP2), a molecule that interacts with  p53 and Bcl2.	transcription
72639	1	336261	7	NULL	NULL	NULL	NULL	p53	GP		required for		consistently			APC	GP	upregulation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_272_49_30619_s_115	9388195	Since we observed a consistent requirement for p53 in APC up-regulation, it appears that a p53-mediated signaling pathway is required for APC regulation in response to DNA damage.	transcription
72640	2	336261	7	NULL	NULL	0	NULL	 p53	GP		mediates					signaling pathway	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_49_30619_s_115	9388195	Since we observed a consistent requirement for p53 in APC up-regulation, it appears that a p53-mediated signaling pathway is required for APC regulation in response to DNA damage.	transcription
72641	3	336261	7	NULL	NULL	0	NULL	statement 2	Process		is required for					APC	GP	regulation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_49_30619_s_115	9388195	Since we observed a consistent requirement for p53 in APC up-regulation, it appears that a p53-mediated signaling pathway is required for APC regulation in response to DNA damage.	transcription
72642	4	336261	7	NULL	NULL	0	NULL	statement 3	Process		in response to					DNA damage	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_49_30619_s_115	9388195	Since we observed a consistent requirement for p53 in APC up-regulation, it appears that a p53-mediated signaling pathway is required for APC regulation in response to DNA damage.	transcription
72643	1	336262	7	NULL	NULL	0	NULL	APC signaling	Process		down-regulates		strongly;;specifically			Thrombospondin-1	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_19808_s_222	15769747	Thrombospondin-1, which was also strongly down-regulated specifically by APC signaling, is a target for positive transcriptional regulation by p53 ( ), suggesting that p53 suppression may be an upstream effector mechanism for protective APC signaling.	transcription
72644	2	336262	7	NULL	NULL	0	NULL	Thrombospondin-1	GP		target for					p53	GP	positive transcriptional regulation by			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_19808_s_222	15769747	Thrombospondin-1, which was also strongly down-regulated specifically by APC signaling, is a target for positive transcriptional regulation by p53 ( ), suggesting that p53 suppression may be an upstream effector mechanism for protective APC signaling.	transcription
72645	3	336262	7	NULL	NULL	0	NULL	p53	GP	suppression of	upstream effector		may be			APC signaling	Process	mechanism for protective			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_19808_s_222	15769747	Thrombospondin-1, which was also strongly down-regulated specifically by APC signaling, is a target for positive transcriptional regulation by p53 ( ), suggesting that p53 suppression may be an upstream effector mechanism for protective APC signaling.	transcription
72646	1	336263	7	NULL	NULL	0	NULL	alkylation	Process		induce					DNA damage	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_49_30619_s_9	9388195	These results support a model featuring a direct link between p53 and APC in response to alkylation-induced DNA damage and suggest a novel role for p53 in a stress-response pathway involving APC.	transcription
72647	2	336263	7	NULL	NULL	0	NULL	stress response pathway	Process		involves					APC	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_49_30619_s_9	9388195	These results support a model featuring a direct link between p53 and APC in response to alkylation-induced DNA damage and suggest a novel role for p53 in a stress-response pathway involving APC.	transcription
72648	3	336263	7	NULL	NULL	0	NULL	p53	GP		play a role in					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_49_30619_s_9	9388195	These results support a model featuring a direct link between p53 and APC in response to alkylation-induced DNA damage and suggest a novel role for p53 in a stress-response pathway involving APC.	transcription
72649	4	336263	7	NULL	NULL	0	NULL	p53	GP		linked to		directly			APC	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_49_30619_s_9	9388195	These results support a model featuring a direct link between p53 and APC in response to alkylation-induced DNA damage and suggest a novel role for p53 in a stress-response pathway involving APC.	transcription
72650	5	336263	7	NULL	NULL	0	NULL	statement 4	Process		in response to					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_49_30619_s_9	9388195	These results support a model featuring a direct link between p53 and APC in response to alkylation-induced DNA damage and suggest a novel role for p53 in a stress-response pathway involving APC.	transcription
72651	1	336264	7	NULL	NULL	0	NULL	APC	GP	induction of;;wildtype	reduce					DNMT1 message	Process				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_24_1_17_s_149	12538344	Further reduction of  DNMT1 message, to almost 34% of that with p53 expression alone, was effected by induction of wildtype APC (Figure 4B,D).	transcription
72652	2	336264	7	NULL	NULL	0	NULL	statement 1	Process		occur with					p53	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_24_1_17_s_149	12538344	Further reduction of  DNMT1 message, to almost 34% of that with p53 expression alone, was effected by induction of wildtype APC (Figure 4B,D).	transcription
72653	1	336265	7	NULL	NULL	NULL	NULL	RXR	GP		regulates					beta-Catenin pathway	GP	degradation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_32_29954_s_191	12771132	The RXR-regulatedbeta -Catenin Degradation Pathway Is  Independent of the p53/ Siah-1- and GSK3beta -regulated APC  Pathways --	transcription
72654	2	336265	7	NULL	NULL	0	NULL	p53/ Siah-1	GP		regulates					APC pathway	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_32_29954_s_191	12771132	The RXR-regulatedbeta -Catenin Degradation Pathway Is  Independent of the p53/ Siah-1- and GSK3beta -regulated APC  Pathways --	transcription
72655	3	336265	7	NULL	NULL	0	NULL	GSK3beta	GP		regulates					APC pathway	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_32_29954_s_191	12771132	The RXR-regulatedbeta -Catenin Degradation Pathway Is  Independent of the p53/ Siah-1- and GSK3beta -regulated APC  Pathways --	transcription
72656	4	336265	7	NULL	NULL	0	NULL	statement 1	Process		is independent of					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_32_29954_s_191	12771132	The RXR-regulatedbeta -Catenin Degradation Pathway Is  Independent of the p53/ Siah-1- and GSK3beta -regulated APC  Pathways --	transcription
72657	5	336265	7	NULL	NULL	0	NULL	statement 1	Process		is independent of					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_32_29954_s_191	12771132	The RXR-regulatedbeta -Catenin Degradation Pathway Is  Independent of the p53/ Siah-1- and GSK3beta -regulated APC  Pathways --	transcription
72658	1	336266	7	NULL	NULL	0	NULL	 p53	GP		regulates		positively			TSP-1	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_pnas_100_22_12718_s_17	14555767	It has been previously shown that TSP-1 expression is positively regulated by the p53, PTEN, Smad, and APC tumor suppressor proteins (  -  ).	transcription
72659	2	336266	7	NULL	NULL	0	NULL	PTEN	GP		regulates		positively			TSP-1	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_pnas_100_22_12718_s_17	14555767	It has been previously shown that TSP-1 expression is positively regulated by the p53, PTEN, Smad, and APC tumor suppressor proteins (  -  ).	transcription
72660	3	336266	7	NULL	NULL	0	NULL	 Smad	GP		regulates		positively			TSP-1	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_pnas_100_22_12718_s_17	14555767	It has been previously shown that TSP-1 expression is positively regulated by the p53, PTEN, Smad, and APC tumor suppressor proteins (  -  ).	transcription
72661	4	336266	7	NULL	NULL	0	NULL	APC tumor suppressor proteins	GP		regulates		positively			TSP-1	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_pnas_100_22_12718_s_17	14555767	It has been previously shown that TSP-1 expression is positively regulated by the p53, PTEN, Smad, and APC tumor suppressor proteins (  -  ).	transcription
72662	1	336267	7	NULL	NULL	0	NULL	 Apc	GP	mutation of	cause					apoptosis	Process	resistance to			NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_22_5_821_s_109	11323404	Curcumin treatment may inhibit apoptosis resistance associated with  Apc mutation through alteration of the equilibrium of NFkappaB and p53.	transcription
72663	2	336267	7	NULL	NULL	0	NULL	curcumin	Chemical		inhibit		may			statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_22_5_821_s_109	11323404	Curcumin treatment may inhibit apoptosis resistance associated with  Apc mutation through alteration of the equilibrium of NFkappaB and p53.	transcription
72664	3	336267	7	NULL	NULL	0	NULL	statement 1	Process		occur through					NFkappaB	GP	alteration of;;equilibrium of			NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_22_5_821_s_109	11323404	Curcumin treatment may inhibit apoptosis resistance associated with  Apc mutation through alteration of the equilibrium of NFkappaB and p53.	transcription
72665	4	336267	7	NULL	NULL	0	NULL	statement 1	Process		occur through					p53	GP	alteration of;;equilibrium of			NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_22_5_821_s_109	11323404	Curcumin treatment may inhibit apoptosis resistance associated with  Apc mutation through alteration of the equilibrium of NFkappaB and p53.	transcription
72666	1	336268	7	NULL	NULL	0	NULL	p53	GP		downregulates					beta-Catenin	GP				NULL		0	NULL	NULL	NULL	gw60_cell_105_5_563_s_68	11389825	Dominant negative versions  of SIP, Ebi, and the C-terminal fragment of APC  also inhibited the downregulation of beta-catenin by  p53.	transcription
72667	2	336268	7	NULL	NULL	0	NULL	SIP	GP	dominant negative versions of	inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_cell_105_5_563_s_68	11389825	Dominant negative versions  of SIP, Ebi, and the C-terminal fragment of APC  also inhibited the downregulation of beta-catenin by  p53.	transcription
72668	3	336268	7	NULL	NULL	0	NULL	Ebi	GP	dominant negative versions of	inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_cell_105_5_563_s_68	11389825	Dominant negative versions  of SIP, Ebi, and the C-terminal fragment of APC  also inhibited the downregulation of beta-catenin by  p53.	transcription
72669	4	336268	7	NULL	NULL	0	NULL	APC	GP	dominant negative versions of	inhibit			C-terminal fragment of		statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_cell_105_5_563_s_68	11389825	Dominant negative versions  of SIP, Ebi, and the C-terminal fragment of APC  also inhibited the downregulation of beta-catenin by  p53.	transcription
72670	1	336269	7	NULL	NULL	0	NULL	 Siah-1	GP		induces					beta-Catenin	GP	degradation of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_11_3803_s_401	11997515	It has recently been reported that Siah-1 induces the degradation of beta-catenin through APC in response to p53 ( 36,  38).	transcription
72671	2	336269	7	NULL	NULL	0	NULL	statement 1	Process		occur through					APC	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_11_3803_s_401	11997515	It has recently been reported that Siah-1 induces the degradation of beta-catenin through APC in response to p53 ( 36,  38).	transcription
72672	3	336269	7	NULL	NULL	0	NULL	statement 1	Process		in response to					p53	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_22_11_3803_s_401	11997515	It has recently been reported that Siah-1 induces the degradation of beta-catenin through APC in response to p53 ( 36,  38).	transcription
72673	1	336270	7	NULL	NULL	0	NULL	p53 protein	GP	increase in levels of	required for					APC gene	GP	expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_49_30619_s_102	9388195	These results demonstrate that an increase in p53 protein level is required for  APC gene expression after DNA damage.	transcription
72674	2	336270	7	NULL	NULL	0	NULL	statement 1	Process		occur after					DNA damage	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_49_30619_s_102	9388195	These results demonstrate that an increase in p53 protein level is required for  APC gene expression after DNA damage.	transcription
72675	1	336271	7	NULL	NULL	0	NULL	Apc	GP		interacts with					p53	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_97_7_3461_s_19	10716720	Does an interaction between  Apc and  p53 affect intestinal neoplasia in experimental models of cancer ( 6)?	transcription
72676	1	336272	7	NULL	NULL	0	NULL	Apc	GP	loss of	induce					apoptosis	Process				NULL	 neural crest-derived cells	0	NULL	NULL	NULL	gw60_pnas_99_1_297_s_167	11756652	These data strongly indicate that the apoptosis of neural crest-derived cells induced by the loss of Apc was not mediated by p53.	transcription
72677	2	336272	7	NULL	NULL	0	NULL	statement 1	Process		is not mediated by					p53	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_99_1_297_s_167	11756652	These data strongly indicate that the apoptosis of neural crest-derived cells induced by the loss of Apc was not mediated by p53.	transcription
72678	1	336273	7	NULL	NULL	0	NULL	MTS-1	GP		encode					p16	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_94_3_952_s_17	9023363	They include  Rb,  p53,  WT1,  BRCA1,  BRCA2,  VHL,  APC,  NF-1,  NF-2, and  MTS-1 (encodes p16, a cell cycle inhibitor).	transcription
72679	2	336273	7	NULL	NULL	0	NULL	p16	GP		is a inhibitor of					cell cycle 	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_94_3_952_s_17	9023363	They include  Rb,  p53,  WT1,  BRCA1,  BRCA2,  VHL,  APC,  NF-1,  NF-2, and  MTS-1 (encodes p16, a cell cycle inhibitor).	transcription
72680	1	336274	7	NULL	NULL	NULL	NULL	DMH	Chemical		induce					CRC susceptibility loci	Chromosome				NULL	recombinant congenic mice	NULL	NULL	NULL	NULL	gw60_pnas_94_7_3308_s_29	9096389	In support of this, DMH-induced CRC susceptibility loci mapped in recombinant congenic mice do not appear to involve  Apc or  P53 ( 10).	transcription
72681	2	336274	7	NULL	NULL	0	NULL	statement 1	Process		does not involve					Apc	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_94_7_3308_s_29	9096389	In support of this, DMH-induced CRC susceptibility loci mapped in recombinant congenic mice do not appear to involve  Apc or  P53 ( 10).	transcription
72682	3	336274	7	NULL	NULL	0	NULL	statement 1	Process		does not involve					p53	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_94_7_3308_s_29	9096389	In support of this, DMH-induced CRC susceptibility loci mapped in recombinant congenic mice do not appear to involve  Apc or  P53 ( 10).	transcription
72683	1	336275	7	NULL	NULL	0	NULL	APC	GP	intact/functional	required for					beta-Catenin	GP	suppression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_34_35583_s_225	15190077	Because a recent report suggested that intact/functional APC was required for the suppression of beta-catenin levels and colon carcinogenesis following PPARgamma activation ( ), we determined whether PPARgamma-mediated suppression of beta-catenin involved APC and p53.	transcription
72684	2	336275	7	NULL	NULL	0	NULL	APC	GP	intact/functional	required for					colon carcinogenesis	Process	suppression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_34_35583_s_225	15190077	Because a recent report suggested that intact/functional APC was required for the suppression of beta-catenin levels and colon carcinogenesis following PPARgamma activation ( ), we determined whether PPARgamma-mediated suppression of beta-catenin involved APC and p53.	transcription
72685	3	336275	7	NULL	NULL	0	NULL	statement 1	Process		occur upon					PPARgamma	GP	activation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_34_35583_s_225	15190077	Because a recent report suggested that intact/functional APC was required for the suppression of beta-catenin levels and colon carcinogenesis following PPARgamma activation ( ), we determined whether PPARgamma-mediated suppression of beta-catenin involved APC and p53.	transcription
72686	4	336275	7	NULL	NULL	0	NULL	statement 1	Process		required for					colon carcinogenesis	Process	activation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_34_35583_s_225	15190077	Because a recent report suggested that intact/functional APC was required for the suppression of beta-catenin levels and colon carcinogenesis following PPARgamma activation ( ), we determined whether PPARgamma-mediated suppression of beta-catenin involved APC and p53.	transcription
72687	5	336275	7	NULL	NULL	0	NULL	PPARgamma	GP		mediate					beta-catenin	GP	suppression of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_34_35583_s_225	15190077	Because a recent report suggested that intact/functional APC was required for the suppression of beta-catenin levels and colon carcinogenesis following PPARgamma activation ( ), we determined whether PPARgamma-mediated suppression of beta-catenin involved APC and p53.	transcription
72688	1	336276	7	NULL	NULL	0	NULL	p53	GP	expression of	regulate					APC gene	GP	expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_49_30619_s_109	9388195	The results show that  APC mRNA levels were increased in a dose-dependent manner in CMV-p53-transfected  versus untransfected K562 cells (Fig.  4 B), clearly indicating that p53 expression can regulate  APC gene expression.	transcription
72689	1	336277	7	NULL	NULL	0	NULL	APC/Apc	GP		is involved in					neoplasia	MedicalFinding	controlling			NULL		0	NULL	NULL	NULL	gw60_pnas_97_7_3461_s_176	10716720	Beyond the negative regulatory genes of neoplasia,  APC/Apc and  p53, the modifier gene  Mom1 encoding the secretory phospholipase Pla2g2a and the pharmacological agents piroxicam and DFMO must be placed in the network of interactions controlling neoplasia.	transcription
72690	2	336277	7	NULL	NULL	0	NULL	p53	GP		is involved in					neoplasia	MedicalFinding	controlling			NULL		0	NULL	NULL	NULL	gw60_pnas_97_7_3461_s_176	10716720	Beyond the negative regulatory genes of neoplasia,  APC/Apc and  p53, the modifier gene  Mom1 encoding the secretory phospholipase Pla2g2a and the pharmacological agents piroxicam and DFMO must be placed in the network of interactions controlling neoplasia.	transcription
72691	3	336277	7	NULL	NULL	0	NULL	Mom1	GP		encode					Pla2g2a	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_97_7_3461_s_176	10716720	Beyond the negative regulatory genes of neoplasia,  APC/Apc and  p53, the modifier gene  Mom1 encoding the secretory phospholipase Pla2g2a and the pharmacological agents piroxicam and DFMO must be placed in the network of interactions controlling neoplasia.	transcription
72692	4	336277	7	NULL	NULL	0	NULL	Mom1	GP		is involved in					neoplasia	MedicalFinding	controlling			NULL		0	NULL	NULL	NULL	gw60_pnas_97_7_3461_s_176	10716720	Beyond the negative regulatory genes of neoplasia,  APC/Apc and  p53, the modifier gene  Mom1 encoding the secretory phospholipase Pla2g2a and the pharmacological agents piroxicam and DFMO must be placed in the network of interactions controlling neoplasia.	transcription
72693	5	336277	7	NULL	NULL	0	NULL	piroxicam 	Chemical		is involved in					neoplasia	MedicalFinding	controlling			NULL		0	NULL	NULL	NULL	gw60_pnas_97_7_3461_s_176	10716720	Beyond the negative regulatory genes of neoplasia,  APC/Apc and  p53, the modifier gene  Mom1 encoding the secretory phospholipase Pla2g2a and the pharmacological agents piroxicam and DFMO must be placed in the network of interactions controlling neoplasia.	transcription
72694	6	336277	7	NULL	NULL	0	NULL	DFMO	Chemical		is involved in					neoplasia	MedicalFinding	controlling			NULL		0	NULL	NULL	NULL	gw60_pnas_97_7_3461_s_176	10716720	Beyond the negative regulatory genes of neoplasia,  APC/Apc and  p53, the modifier gene  Mom1 encoding the secretory phospholipase Pla2g2a and the pharmacological agents piroxicam and DFMO must be placed in the network of interactions controlling neoplasia.	transcription
72695	7	336277	7	NULL	NULL	0	NULL	 Mom1	GP		is a type of					modifier gene	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_97_7_3461_s_176	10716720	Beyond the negative regulatory genes of neoplasia,  APC/Apc and  p53, the modifier gene  Mom1 encoding the secretory phospholipase Pla2g2a and the pharmacological agents piroxicam and DFMO must be placed in the network of interactions controlling neoplasia.	transcription
72696	8	336277	7	NULL	NULL	0	NULL	Pla2g2a	GP		is a type of					secretory phospholipase	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_97_7_3461_s_176	10716720	Beyond the negative regulatory genes of neoplasia,  APC/Apc and  p53, the modifier gene  Mom1 encoding the secretory phospholipase Pla2g2a and the pharmacological agents piroxicam and DFMO must be placed in the network of interactions controlling neoplasia.	transcription
72697	9	336277	7	NULL	NULL	0	NULL	piroxicam	Chemical		is a type of					pharmacological agent	Chemical				NULL		0	NULL	NULL	NULL	gw60_pnas_97_7_3461_s_176	10716720	Beyond the negative regulatory genes of neoplasia,  APC/Apc and  p53, the modifier gene  Mom1 encoding the secretory phospholipase Pla2g2a and the pharmacological agents piroxicam and DFMO must be placed in the network of interactions controlling neoplasia.	transcription
72698	10	336277	7	NULL	NULL	0	NULL	DFMO	Chemical		is a type of					pharmacological agent	Chemical				NULL		0	NULL	NULL	NULL	gw60_pnas_97_7_3461_s_176	10716720	Beyond the negative regulatory genes of neoplasia,  APC/Apc and  p53, the modifier gene  Mom1 encoding the secretory phospholipase Pla2g2a and the pharmacological agents piroxicam and DFMO must be placed in the network of interactions controlling neoplasia.	transcription
72699	1	336278	7	NULL	NULL	0	NULL	p53BP-2	GP		interact with					Bcl-2	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_17_14514_s_47	11278422	Like p53, p53BP-2 is part of a protein network since it has been shown that p53BP-2 can also interact with Bcl-2 (an anti-apoptotic protein), protein phosphatase-1gamma, NF-kappaB subunit p65 (a transcription factor), and APCL ( adenomatous  polyposis  coli- like) protein (a tumor suppressor-like protein) ( 19-22).	transcription
72700	2	336278	7	NULL	NULL	0	NULL	p53BP-2	GP		interacts with					protein phosphatase-1gamma	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_17_14514_s_47	11278422	Like p53, p53BP-2 is part of a protein network since it has been shown that p53BP-2 can also interact with Bcl-2 (an anti-apoptotic protein), protein phosphatase-1gamma, NF-kappaB subunit p65 (a transcription factor), and APCL ( adenomatous  polyposis  coli- like) protein (a tumor suppressor-like protein) ( 19-22).	transcription
72701	3	336278	7	NULL	NULL	0	NULL	p53BP-2	GP		interacts with					p65	GP		NF-kappaB subunit 		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_17_14514_s_47	11278422	Like p53, p53BP-2 is part of a protein network since it has been shown that p53BP-2 can also interact with Bcl-2 (an anti-apoptotic protein), protein phosphatase-1gamma, NF-kappaB subunit p65 (a transcription factor), and APCL ( adenomatous  polyposis  coli- like) protein (a tumor suppressor-like protein) ( 19-22).	transcription
72702	4	336278	7	NULL	NULL	NULL	NULL	p53BP-2	GP		interacts with					APCL	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_17_14514_s_47	11278422	Like p53, p53BP-2 is part of a protein network since it has been shown that p53BP-2 can also interact with Bcl-2 (an anti-apoptotic protein), protein phosphatase-1gamma, NF-kappaB subunit p65 (a transcription factor), and APCL ( adenomatous  polyposis  coli- like) protein (a tumor suppressor-like protein) ( 19-22).	transcription
72703	5	336278	7	NULL	NULL	0	NULL	Bcl-2	GP		is a type of					anti-apoptotic protein	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_17_14514_s_47	11278422	Like p53, p53BP-2 is part of a protein network since it has been shown that p53BP-2 can also interact with Bcl-2 (an anti-apoptotic protein), protein phosphatase-1gamma, NF-kappaB subunit p65 (a transcription factor), and APCL ( adenomatous  polyposis  coli- like) protein (a tumor suppressor-like protein) ( 19-22).	transcription
72704	6	336278	7	NULL	NULL	0	NULL	p65	GP		is a type of					transcription factor	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_17_14514_s_47	11278422	Like p53, p53BP-2 is part of a protein network since it has been shown that p53BP-2 can also interact with Bcl-2 (an anti-apoptotic protein), protein phosphatase-1gamma, NF-kappaB subunit p65 (a transcription factor), and APCL ( adenomatous  polyposis  coli- like) protein (a tumor suppressor-like protein) ( 19-22).	transcription
72705	7	336278	7	NULL	NULL	0	NULL	APCL	GP		is					adenomatous polyposis coli- like	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_17_14514_s_47	11278422	Like p53, p53BP-2 is part of a protein network since it has been shown that p53BP-2 can also interact with Bcl-2 (an anti-apoptotic protein), protein phosphatase-1gamma, NF-kappaB subunit p65 (a transcription factor), and APCL ( adenomatous  polyposis  coli- like) protein (a tumor suppressor-like protein) ( 19-22).	transcription
72706	8	336278	7	NULL	NULL	0	NULL	APCL	GP		is a type of					tumor suppressor-like protein	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_17_14514_s_47	11278422	Like p53, p53BP-2 is part of a protein network since it has been shown that p53BP-2 can also interact with Bcl-2 (an anti-apoptotic protein), protein phosphatase-1gamma, NF-kappaB subunit p65 (a transcription factor), and APCL ( adenomatous  polyposis  coli- like) protein (a tumor suppressor-like protein) ( 19-22).	transcription
72707	9	336278	7	NULL	NULL	0	NULL	p53BP-2	GP		is like					p53	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_17_14514_s_47	11278422	Like p53, p53BP-2 is part of a protein network since it has been shown that p53BP-2 can also interact with Bcl-2 (an anti-apoptotic protein), protein phosphatase-1gamma, NF-kappaB subunit p65 (a transcription factor), and APCL ( adenomatous  polyposis  coli- like) protein (a tumor suppressor-like protein) ( 19-22).	transcription
72708	1	336279	7	NULL	NULL	0	NULL	 APC	GP		consist of				 promoter	single SP1 consensus sequence	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_64_2_415_s_153	12869646	The APC promoter consists of a single SP1 consensus sequence, possibly  contributing to p53 gene modulation, yet its necessity for p53 stimulation is  undermined by the existing alternate mechanisms (i.e., direct interaction of  p53 with promoter and modulation by a p53 complex with TFIIH)  (Jaiswal and Narayan, 2001  ).	transcription
72709	2	336279	7	NULL	NULL	0	NULL	statement 1	Process		contribute to					p53 gene 	GP	modulation of			NULL		0	NULL	NULL	NULL	gw60_molpharmacol_64_2_415_s_153	12869646	The APC promoter consists of a single SP1 consensus sequence, possibly  contributing to p53 gene modulation, yet its necessity for p53 stimulation is  undermined by the existing alternate mechanisms (i.e., direct interaction of  p53 with promoter and modulation by a p53 complex with TFIIH)  (Jaiswal and Narayan, 2001  ).	transcription
72710	3	336279	7	NULL	NULL	0	NULL	p53	GP		interacts with		directly							promoter	NULL		0	NULL	NULL	NULL	gw60_molpharmacol_64_2_415_s_153	12869646	The APC promoter consists of a single SP1 consensus sequence, possibly  contributing to p53 gene modulation, yet its necessity for p53 stimulation is  undermined by the existing alternate mechanisms (i.e., direct interaction of  p53 with promoter and modulation by a p53 complex with TFIIH)  (Jaiswal and Narayan, 2001  ).	transcription
72711	4	336279	7	NULL	NULL	0	NULL	p53	GP		complex with					TFIIH	GP				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_64_2_415_s_153	12869646	The APC promoter consists of a single SP1 consensus sequence, possibly  contributing to p53 gene modulation, yet its necessity for p53 stimulation is  undermined by the existing alternate mechanisms (i.e., direct interaction of  p53 with promoter and modulation by a p53 complex with TFIIH)  (Jaiswal and Narayan, 2001  ).	transcription
72712	5	336279	7	NULL	NULL	0	NULL	statement 3	Process		modulated by					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_molpharmacol_64_2_415_s_153	12869646	The APC promoter consists of a single SP1 consensus sequence, possibly  contributing to p53 gene modulation, yet its necessity for p53 stimulation is  undermined by the existing alternate mechanisms (i.e., direct interaction of  p53 with promoter and modulation by a p53 complex with TFIIH)  (Jaiswal and Narayan, 2001  ).	transcription
72713	1	336280	7	NULL	NULL	NULL	NULL	Apoptin	GP		induce					G2/M arrest	Process				NULL	p53 null transformed cells	NULL	NULL	NULL	NULL	gw70_genesdev_18_16_1952_s_121	15314021	Our results suggest that Apoptin induces G2/M arrest and apoptosis in p53 null transformed cells through association with and inhibition of the APC/C.	transcription
72714	2	336280	7	NULL	NULL	0	NULL	Apoptin	GP		induce					apoptosis	Process				NULL	p53 null transformed cells	0	NULL	NULL	NULL	gw70_genesdev_18_16_1952_s_121	15314021	Our results suggest that Apoptin induces G2/M arrest and apoptosis in p53 null transformed cells through association with and inhibition of the APC/C.	transcription
72715	3	336280	7	NULL	NULL	0	NULL	statement 1	Process		occur through					APC/C	GP	association with			NULL		0	NULL	NULL	NULL	gw70_genesdev_18_16_1952_s_121	15314021	Our results suggest that Apoptin induces G2/M arrest and apoptosis in p53 null transformed cells through association with and inhibition of the APC/C.	transcription
72716	4	336280	7	NULL	NULL	0	NULL	statement 2	Process		occur through					APC/C	GP	association with			NULL		0	NULL	NULL	NULL	gw70_genesdev_18_16_1952_s_121	15314021	Our results suggest that Apoptin induces G2/M arrest and apoptosis in p53 null transformed cells through association with and inhibition of the APC/C.	transcription
72717	5	336280	7	NULL	NULL	0	NULL	statement 1	Process		occur through					APC/C	GP	inhibition of			NULL		0	NULL	NULL	NULL	gw70_genesdev_18_16_1952_s_121	15314021	Our results suggest that Apoptin induces G2/M arrest and apoptosis in p53 null transformed cells through association with and inhibition of the APC/C.	transcription
72718	6	336280	7	NULL	NULL	0	NULL	statement 2	Process		occur through					APC/C	GP	inhibition of			NULL		0	NULL	NULL	NULL	gw70_genesdev_18_16_1952_s_121	15314021	Our results suggest that Apoptin induces G2/M arrest and apoptosis in p53 null transformed cells through association with and inhibition of the APC/C.	transcription
72719	7	336280	7	NULL	NULL	0	NULL	statement 3	Process		occur along with					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_genesdev_18_16_1952_s_121	15314021	Our results suggest that Apoptin induces G2/M arrest and apoptosis in p53 null transformed cells through association with and inhibition of the APC/C.	transcription
72720	8	336280	7	NULL	NULL	0	NULL	statement 4	Process		occur along with					statement 6	Process				NULL		0	NULL	NULL	NULL	gw70_genesdev_18_16_1952_s_121	15314021	Our results suggest that Apoptin induces G2/M arrest and apoptosis in p53 null transformed cells through association with and inhibition of the APC/C.	transcription
72721	1	336281	7	NULL	NULL	0	NULL	 APC	GP		bind					EPCR	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_19808_s_165	15769747	Antibody-blocking experiments demonstrate that this suppressive effect on p53 expression was dependent on APC binding to EPCR as well as PAR1 cleavage ( Fig. 5 B).	transcription
72722	2	336281	7	NULL	NULL	0	NULL	APC	GP		bind					PAR1 cleavage 	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_19808_s_165	15769747	Antibody-blocking experiments demonstrate that this suppressive effect on p53 expression was dependent on APC binding to EPCR as well as PAR1 cleavage ( Fig. 5 B).	transcription
72723	3	336281	7	NULL	NULL	0	NULL	p53	GP	suppressive effect of	depends on					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_19808_s_165	15769747	Antibody-blocking experiments demonstrate that this suppressive effect on p53 expression was dependent on APC binding to EPCR as well as PAR1 cleavage ( Fig. 5 B).	transcription
72724	4	336281	7	NULL	NULL	NULL	NULL	p53	GP	suppressive effect of	depends on					statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_280_20_19808_s_165	15769747	Antibody-blocking experiments demonstrate that this suppressive effect on p53 expression was dependent on APC binding to EPCR as well as PAR1 cleavage ( Fig. 5 B).	transcription
72725	1	336282	7	NULL	NULL	0	NULL	N-MethylN''-nitro-N-nitrosoguanidine 	Chemical		activates					APC gene	GP	expression of			NULL		0	NULL	NULL	NULL	gw60_cellbiol_136_3_693_s_460	9024698	Activation of Adenomatous Polyposis Coli (APC) Gene Expression by the DNA-alkylating Agent N-MethylN''-nitro-N-nitrosoguanidine Requires p53.	transcription
72726	2	336282	7	NULL	NULL	0	NULL	statement 1	Process		requires					p53	GP				NULL		0	NULL	NULL	NULL	gw60_cellbiol_136_3_693_s_460	9024698	Activation of Adenomatous Polyposis Coli (APC) Gene Expression by the DNA-alkylating Agent N-MethylN''-nitro-N-nitrosoguanidine Requires p53.	transcription
72727	3	336282	7	NULL	NULL	0	NULL	APC	Organism		is					Adenomatous Polyposis Coli	Organism				NULL		0	NULL	NULL	NULL	gw60_cellbiol_136_3_693_s_460	9024698	Activation of Adenomatous Polyposis Coli (APC) Gene Expression by the DNA-alkylating Agent N-MethylN''-nitro-N-nitrosoguanidine Requires p53.	transcription
72728	4	336282	7	NULL	NULL	0	NULL	N-MethylN''-nitro-N-nitrosoguanidine	Chemical		is a type of					DNA-alkylating Agent	Chemical				NULL		0	NULL	NULL	NULL	gw60_cellbiol_136_3_693_s_460	9024698	Activation of Adenomatous Polyposis Coli (APC) Gene Expression by the DNA-alkylating Agent N-MethylN''-nitro-N-nitrosoguanidine Requires p53.	transcription
72729	1	336283	7	NULL	NULL	0	NULL	APC gene	GP	inactivation of	during					adenoma	MedicalFinding	development of			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_306_4_799_s_66	12821112	In this sequence, the APC gene (5q) is inactivated  at an early stage, followed by activation of the K-ras gene during the development  of moderate to severe adenoma, and inactivation of the p53 gene (17p) at the stage  of conversion from adenoma to carcinoma.	transcription
72730	2	336283	7	NULL	NULL	0	NULL	statement 1	Process		followed by					K-ras gene	GP	activation of			NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_306_4_799_s_66	12821112	In this sequence, the APC gene (5q) is inactivated  at an early stage, followed by activation of the K-ras gene during the development  of moderate to severe adenoma, and inactivation of the p53 gene (17p) at the stage  of conversion from adenoma to carcinoma.	transcription
72731	3	336283	7	NULL	NULL	0	NULL	adenoma	MedicalFinding		converted to					carcinoma	MedicalFinding				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_306_4_799_s_66	12821112	In this sequence, the APC gene (5q) is inactivated  at an early stage, followed by activation of the K-ras gene during the development  of moderate to severe adenoma, and inactivation of the p53 gene (17p) at the stage  of conversion from adenoma to carcinoma.	transcription
72732	4	336283	7	NULL	NULL	0	NULL	p53 gene	GP	inactivation of	occur during					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_biochmbiophyrescomm_306_4_799_s_66	12821112	In this sequence, the APC gene (5q) is inactivated  at an early stage, followed by activation of the K-ras gene during the development  of moderate to severe adenoma, and inactivation of the p53 gene (17p) at the stage  of conversion from adenoma to carcinoma.	transcription
72733	1	336284	7	NULL	NULL	0	NULL	APC gene	GP		is					inducible	Process				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_27_2_252_s_31	16150893	We also found that the  APC gene is inducible, and its expression can be regulated by DNA-alkylating agent  N-methyl- N''-nitro- N-nitrosoguanidine (MNNG), which is mediated by p53 (   -  ).	transcription
72734	2	336284	7	NULL	NULL	NULL	NULL	MNNG	Chemical		regulates					APC gene	GP	expression of			NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_2_252_s_31	16150893	We also found that the  APC gene is inducible, and its expression can be regulated by DNA-alkylating agent  N-methyl- N''-nitro- N-nitrosoguanidine (MNNG), which is mediated by p53 (   -  ).	transcription
72735	3	336284	7	NULL	NULL	0	NULL	statement 2	Process		mediated by					p53	GP				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_27_2_252_s_31	16150893	We also found that the  APC gene is inducible, and its expression can be regulated by DNA-alkylating agent  N-methyl- N''-nitro- N-nitrosoguanidine (MNNG), which is mediated by p53 (   -  ).	transcription
72736	4	336284	7	NULL	NULL	0	NULL	MNNG	Chemical		is					N-methyl- N''-nitro- N-nitrosoguanidine	Chemical				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_27_2_252_s_31	16150893	We also found that the  APC gene is inducible, and its expression can be regulated by DNA-alkylating agent  N-methyl- N''-nitro- N-nitrosoguanidine (MNNG), which is mediated by p53 (   -  ).	transcription
72737	5	336284	7	NULL	NULL	0	NULL	MNNG	Chemical		is a type of					DNA-alkylating agent	Chemical				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_27_2_252_s_31	16150893	We also found that the  APC gene is inducible, and its expression can be regulated by DNA-alkylating agent  N-methyl- N''-nitro- N-nitrosoguanidine (MNNG), which is mediated by p53 (   -  ).	transcription
72738	1	336285	7	NULL	NULL	0	NULL	Apc	GP		initiate					intestinal tumor formation	MedicalFinding				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_17_7598_s_339	15314168	The loss of a single allele of the cyclin-dependent kinase inhibitor p21CIP1 also promoted  Apc-initiated intestinal tumor formation ( ), and the loss of a single  p27KIP1 allele ( ), or  p53, which is a regulator of p21CIP1 expression, also promotes tumor formation ( ).	transcription
72739	2	336285	7	NULL	NULL	NULL	NULL	p21CIP1 allele	GP	loss of single 	promote					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_17_7598_s_339	15314168	The loss of a single allele of the cyclin-dependent kinase inhibitor p21CIP1 also promoted  Apc-initiated intestinal tumor formation ( ), and the loss of a single  p27KIP1 allele ( ), or  p53, which is a regulator of p21CIP1 expression, also promotes tumor formation ( ).	transcription
72740	3	336285	7	NULL	NULL	0	NULL	 p27KIP1 allele	GP	loss of single	promote					tumor formation	MedicalFinding				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_17_7598_s_339	15314168	The loss of a single allele of the cyclin-dependent kinase inhibitor p21CIP1 also promoted  Apc-initiated intestinal tumor formation ( ), and the loss of a single  p27KIP1 allele ( ), or  p53, which is a regulator of p21CIP1 expression, also promotes tumor formation ( ).	transcription
72741	4	336285	7	NULL	NULL	0	NULL	p53	GP		regulate					p21CIP1	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_17_7598_s_339	15314168	The loss of a single allele of the cyclin-dependent kinase inhibitor p21CIP1 also promoted  Apc-initiated intestinal tumor formation ( ), and the loss of a single  p27KIP1 allele ( ), or  p53, which is a regulator of p21CIP1 expression, also promotes tumor formation ( ).	transcription
72742	5	336285	7	NULL	NULL	0	NULL	p53	GP		promote					tumor formation	MedicalFinding				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_17_7598_s_339	15314168	The loss of a single allele of the cyclin-dependent kinase inhibitor p21CIP1 also promoted  Apc-initiated intestinal tumor formation ( ), and the loss of a single  p27KIP1 allele ( ), or  p53, which is a regulator of p21CIP1 expression, also promotes tumor formation ( ).	transcription
72743	6	336285	7	NULL	NULL	0	NULL	p21CIP1	GP		is a type of					cyclin-dependent kinase inhibitor	GP				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_17_7598_s_339	15314168	The loss of a single allele of the cyclin-dependent kinase inhibitor p21CIP1 also promoted  Apc-initiated intestinal tumor formation ( ), and the loss of a single  p27KIP1 allele ( ), or  p53, which is a regulator of p21CIP1 expression, also promotes tumor formation ( ).	transcription
72744	7	336285	7	NULL	NULL	0	NULL	statement 2	Process		is an alternative to					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_17_7598_s_339	15314168	The loss of a single allele of the cyclin-dependent kinase inhibitor p21CIP1 also promoted  Apc-initiated intestinal tumor formation ( ), and the loss of a single  p27KIP1 allele ( ), or  p53, which is a regulator of p21CIP1 expression, also promotes tumor formation ( ).	transcription
72746	1	336286	7	NULL	NULL	0	NULL	Mdm2	GP		mediate					ubiquitin/proteasome mechanism	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_11_10615_s_170	14688278	To rule out the possibility that Z-LLal directly inhibits proteasome function, we examined the effect of Z-LLal on the stability of p53 protein, which is known to be degraded by an Mdm2-mediated ubiquitin/proteasome mechanism but not by the APC-dependent pathway.	transcription
72747	2	336286	7	NULL	NULL	0	NULL	p53 protein	GP		not degraded by					APC-dependent pathway	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_11_10615_s_170	14688278	To rule out the possibility that Z-LLal directly inhibits proteasome function, we examined the effect of Z-LLal on the stability of p53 protein, which is known to be degraded by an Mdm2-mediated ubiquitin/proteasome mechanism but not by the APC-dependent pathway.	transcription
72748	3	336286	7	NULL	NULL	0	NULL	p53 protein	GP		degraded by					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_11_10615_s_170	14688278	To rule out the possibility that Z-LLal directly inhibits proteasome function, we examined the effect of Z-LLal on the stability of p53 protein, which is known to be degraded by an Mdm2-mediated ubiquitin/proteasome mechanism but not by the APC-dependent pathway.	transcription
72749	1	336287	7	NULL	NULL	0	NULL	p53	GP		down-regulate					beta-catenin	GP	wt			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_20_6768_s_233	11564862	While p53 could down-regulate wt beta-catenin in the presence of wt or even mutant APC, it failed to affect mutants of beta-catenin that are resistant to the APC-GSK3beta-axin-mediated degradation.	transcription
72750	2	336287	7	NULL	NULL	0	NULL	statement 1	Process		in the presence of					APC	GP	wt			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_20_6768_s_233	11564862	While p53 could down-regulate wt beta-catenin in the presence of wt or even mutant APC, it failed to affect mutants of beta-catenin that are resistant to the APC-GSK3beta-axin-mediated degradation.	transcription
72751	3	336287	7	NULL	NULL	0	NULL	statement 1	Process		in the presence of					APC	GP	mutant			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_20_6768_s_233	11564862	While p53 could down-regulate wt beta-catenin in the presence of wt or even mutant APC, it failed to affect mutants of beta-catenin that are resistant to the APC-GSK3beta-axin-mediated degradation.	transcription
72752	4	336287	7	NULL	NULL	0	NULL	APC-GSK3beta-axin	Process		mediate					beta-catenin	GP	degradation of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_20_6768_s_233	11564862	While p53 could down-regulate wt beta-catenin in the presence of wt or even mutant APC, it failed to affect mutants of beta-catenin that are resistant to the APC-GSK3beta-axin-mediated degradation.	transcription
72753	5	336287	7	NULL	NULL	NULL	NULL	beta-catenin	GP	mutant	resistant to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_20_6768_s_233	11564862	While p53 could down-regulate wt beta-catenin in the presence of wt or even mutant APC, it failed to affect mutants of beta-catenin that are resistant to the APC-GSK3beta-axin-mediated degradation.	transcription
72754	6	336287	7	NULL	NULL	0	NULL	p53	GP		failed to affect					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_20_6768_s_233	11564862	While p53 could down-regulate wt beta-catenin in the presence of wt or even mutant APC, it failed to affect mutants of beta-catenin that are resistant to the APC-GSK3beta-axin-mediated degradation.	transcription
72755	1	336288	7	NULL	NULL	0	NULL	BRCA1	GP		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_23_16582_s_323	10347224	Many well described tumor suppressor/growth arrest genes, such as  BRCA1 ( 55),  APC ( 56),  p53 ( 57),  p33 ING1 ( 58),  CHOP ( 59), and the cyclin-dependent kinase inhibitor  p27 ( 45), also induce apoptosis.	transcription
72756	2	336288	7	NULL	NULL	0	NULL	APC	GP		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_23_16582_s_323	10347224	Many well described tumor suppressor/growth arrest genes, such as  BRCA1 ( 55),  APC ( 56),  p53 ( 57),  p33 ING1 ( 58),  CHOP ( 59), and the cyclin-dependent kinase inhibitor  p27 ( 45), also induce apoptosis.	transcription
72757	3	336288	7	NULL	NULL	0	NULL	p53	GP		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_23_16582_s_323	10347224	Many well described tumor suppressor/growth arrest genes, such as  BRCA1 ( 55),  APC ( 56),  p53 ( 57),  p33 ING1 ( 58),  CHOP ( 59), and the cyclin-dependent kinase inhibitor  p27 ( 45), also induce apoptosis.	transcription
72758	4	336288	7	NULL	NULL	NULL	NULL	p33 ING1	GP		induce					apoptosis	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_23_16582_s_323	10347224	Many well described tumor suppressor/growth arrest genes, such as  BRCA1 ( 55),  APC ( 56),  p53 ( 57),  p33 ING1 ( 58),  CHOP ( 59), and the cyclin-dependent kinase inhibitor  p27 ( 45), also induce apoptosis.	transcription
72759	5	336288	7	NULL	NULL	0	NULL	CHOP	GP		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_23_16582_s_323	10347224	Many well described tumor suppressor/growth arrest genes, such as  BRCA1 ( 55),  APC ( 56),  p53 ( 57),  p33 ING1 ( 58),  CHOP ( 59), and the cyclin-dependent kinase inhibitor  p27 ( 45), also induce apoptosis.	transcription
72760	6	336288	7	NULL	NULL	0	NULL	p27	GP		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_23_16582_s_323	10347224	Many well described tumor suppressor/growth arrest genes, such as  BRCA1 ( 55),  APC ( 56),  p53 ( 57),  p33 ING1 ( 58),  CHOP ( 59), and the cyclin-dependent kinase inhibitor  p27 ( 45), also induce apoptosis.	transcription
72761	7	336288	7	NULL	NULL	0	NULL	BRCA1	GP		is a type of					 tumor suppressor/growth arrest genes	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_23_16582_s_323	10347224	Many well described tumor suppressor/growth arrest genes, such as  BRCA1 ( 55),  APC ( 56),  p53 ( 57),  p33 ING1 ( 58),  CHOP ( 59), and the cyclin-dependent kinase inhibitor  p27 ( 45), also induce apoptosis.	transcription
72762	8	336288	7	NULL	NULL	0	NULL	APC	GP		is a type of					tumor suppressor/growth arrest genes	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_23_16582_s_323	10347224	Many well described tumor suppressor/growth arrest genes, such as  BRCA1 ( 55),  APC ( 56),  p53 ( 57),  p33 ING1 ( 58),  CHOP ( 59), and the cyclin-dependent kinase inhibitor  p27 ( 45), also induce apoptosis.	transcription
72763	9	336288	7	NULL	NULL	0	NULL	p53	GP		is a type of					tumor suppressor/growth arrest genes	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_23_16582_s_323	10347224	Many well described tumor suppressor/growth arrest genes, such as  BRCA1 ( 55),  APC ( 56),  p53 ( 57),  p33 ING1 ( 58),  CHOP ( 59), and the cyclin-dependent kinase inhibitor  p27 ( 45), also induce apoptosis.	transcription
72764	10	336288	7	NULL	NULL	0	NULL	p33 ING1	GP		is a type of					tumor suppressor/growth arrest genes	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_23_16582_s_323	10347224	Many well described tumor suppressor/growth arrest genes, such as  BRCA1 ( 55),  APC ( 56),  p53 ( 57),  p33 ING1 ( 58),  CHOP ( 59), and the cyclin-dependent kinase inhibitor  p27 ( 45), also induce apoptosis.	transcription
72765	11	336288	7	NULL	NULL	0	NULL	CHOP	GP		is a type of					tumor suppressor/growth arrest genes	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_23_16582_s_323	10347224	Many well described tumor suppressor/growth arrest genes, such as  BRCA1 ( 55),  APC ( 56),  p53 ( 57),  p33 ING1 ( 58),  CHOP ( 59), and the cyclin-dependent kinase inhibitor  p27 ( 45), also induce apoptosis.	transcription
72766	12	336288	7	NULL	NULL	0	NULL	p27	GP		is a type of					tumor suppressor/growth arrest genes	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_23_16582_s_323	10347224	Many well described tumor suppressor/growth arrest genes, such as  BRCA1 ( 55),  APC ( 56),  p53 ( 57),  p33 ING1 ( 58),  CHOP ( 59), and the cyclin-dependent kinase inhibitor  p27 ( 45), also induce apoptosis.	transcription
72767	13	336288	7	NULL	NULL	0	NULL	p27	GP		is a inhibitor of					cyclin-dependent kinase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_23_16582_s_323	10347224	Many well described tumor suppressor/growth arrest genes, such as  BRCA1 ( 55),  APC ( 56),  p53 ( 57),  p33 ING1 ( 58),  CHOP ( 59), and the cyclin-dependent kinase inhibitor  p27 ( 45), also induce apoptosis.	transcription
72768	1	336289	7	NULL	NULL	0	NULL	p53 activity	GP 	lack of 	does not effect					neoplasia	MedicalFinding	intestine			NULL	Min mice heterozygous for the Min nonsense allele of Apc	0	NULL	NULL	NULL	gw60_pnas_97_7_3461_s_20	10716720	Preliminary studies tested whether a lack of  p53 activity affected neoplasia in the intestine of Min (multiple intestinal neoplasia) mice heterozygous for the  Min nonsense allele of  Apc, but no significant effect was observed ( 7-10).	transcription
72769	2	336289	7	NULL	NULL	0	NULL	Min	MedicalFinding		is					multiple intestinal neoplasia	MedicalFinding				NULL		0	NULL	NULL	NULL	gw60_pnas_97_7_3461_s_20	10716720	Preliminary studies tested whether a lack of  p53 activity affected neoplasia in the intestine of Min (multiple intestinal neoplasia) mice heterozygous for the  Min nonsense allele of  Apc, but no significant effect was observed ( 7-10).	transcription
72770	1	336290	7	NULL	NULL	0	NULL	E2F	GP		mediate					transcription	Process				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_cell-cycle_5_14_16861914_s_5	16861914	We propose that loss of  pRb repression of E2F-mediated transcription causing misregulation of  Emi1 and APC/C substrates results in the generation of tetraploidy and  proliferation of genomically unstable cells in the absence of normal p53  function.	transcription
72771	2	336290	7	NULL	NULL	0	NULL	pRb	GP		repress					statement 1	Process				NULL		0	NULL	NULL	NULL	abs-batch0740-0759_cell-cycle_5_14_16861914_s_5	16861914	We propose that loss of  pRb repression of E2F-mediated transcription causing misregulation of  Emi1 and APC/C substrates results in the generation of tetraploidy and  proliferation of genomically unstable cells in the absence of normal p53  function.	transcription
72772	3	336290	7	NULL	NULL	0	NULL	statement 2	Process	loss of	cause					Emi1 substrates	GP	misregulation of			NULL		0	NULL	NULL	NULL	abs-batch0740-0759_cell-cycle_5_14_16861914_s_5	16861914	We propose that loss of  pRb repression of E2F-mediated transcription causing misregulation of  Emi1 and APC/C substrates results in the generation of tetraploidy and  proliferation of genomically unstable cells in the absence of normal p53  function.	transcription
72773	4	336290	7	NULL	NULL	0	NULL	statement 2	Process	loss of	cause					APC/C substrates	GP	misregulation of			NULL		0	NULL	NULL	NULL	abs-batch0740-0759_cell-cycle_5_14_16861914_s_5	16861914	We propose that loss of  pRb repression of E2F-mediated transcription causing misregulation of  Emi1 and APC/C substrates results in the generation of tetraploidy and  proliferation of genomically unstable cells in the absence of normal p53  function.	transcription
72774	5	336290	7	NULL	NULL	0	NULL	statement 3	Process		results in					tetraploidy	Process	generation of			NULL		0	NULL	NULL	NULL	abs-batch0740-0759_cell-cycle_5_14_16861914_s_5	16861914	We propose that loss of  pRb repression of E2F-mediated transcription causing misregulation of  Emi1 and APC/C substrates results in the generation of tetraploidy and  proliferation of genomically unstable cells in the absence of normal p53  function.	transcription
72775	6	336290	7	NULL	NULL	0	NULL	statement 3	Process		results in					genomically unstable cells	Cell	proliferation of			NULL		0	NULL	NULL	NULL	abs-batch0740-0759_cell-cycle_5_14_16861914_s_5	16861914	We propose that loss of  pRb repression of E2F-mediated transcription causing misregulation of  Emi1 and APC/C substrates results in the generation of tetraploidy and  proliferation of genomically unstable cells in the absence of normal p53  function.	transcription
72776	7	336290	7	NULL	NULL	0	NULL	statement 4	Process		results in					tetraploidy	Process	generation of			NULL		0	NULL	NULL	NULL	abs-batch0740-0759_cell-cycle_5_14_16861914_s_5	16861914	We propose that loss of  pRb repression of E2F-mediated transcription causing misregulation of  Emi1 and APC/C substrates results in the generation of tetraploidy and  proliferation of genomically unstable cells in the absence of normal p53  function.	transcription
72777	8	336290	7	NULL	NULL	0	NULL	statement 4	Process		results in					genomically unstable cells	Cell	proliferation of			NULL		0	NULL	NULL	NULL	abs-batch0740-0759_cell-cycle_5_14_16861914_s_5	16861914	We propose that loss of  pRb repression of E2F-mediated transcription causing misregulation of  Emi1 and APC/C substrates results in the generation of tetraploidy and  proliferation of genomically unstable cells in the absence of normal p53  function.	transcription
72778	9	336290	7	NULL	NULL	0	NULL	statement 5	Process		in the absence of					p53 function	Process	normal			NULL		0	NULL	NULL	NULL	abs-batch0740-0759_cell-cycle_5_14_16861914_s_5	16861914	We propose that loss of  pRb repression of E2F-mediated transcription causing misregulation of  Emi1 and APC/C substrates results in the generation of tetraploidy and  proliferation of genomically unstable cells in the absence of normal p53  function.	transcription
72779	10	336290	7	NULL	NULL	0	NULL	statement 6	Process		in the absence of					p53 function	Process	normal			NULL		0	NULL	NULL	NULL	abs-batch0740-0759_cell-cycle_5_14_16861914_s_5	16861914	We propose that loss of  pRb repression of E2F-mediated transcription causing misregulation of  Emi1 and APC/C substrates results in the generation of tetraploidy and  proliferation of genomically unstable cells in the absence of normal p53  function.	transcription
72780	11	336290	7	NULL	NULL	0	NULL	statement 7	Process		in the absence of					p53 function	Process	normal			NULL		0	NULL	NULL	NULL	abs-batch0740-0759_cell-cycle_5_14_16861914_s_5	16861914	We propose that loss of  pRb repression of E2F-mediated transcription causing misregulation of  Emi1 and APC/C substrates results in the generation of tetraploidy and  proliferation of genomically unstable cells in the absence of normal p53  function.	transcription
72781	12	336290	7	NULL	NULL	0	NULL	statement 8	Process		in the absence of					p53 function	Process	normal			NULL		0	NULL	NULL	NULL	abs-batch0740-0759_cell-cycle_5_14_16861914_s_5	16861914	We propose that loss of  pRb repression of E2F-mediated transcription causing misregulation of  Emi1 and APC/C substrates results in the generation of tetraploidy and  proliferation of genomically unstable cells in the absence of normal p53  function.	transcription
72782	1	336291	7	NULL	NULL	0	NULL	DMH	Chemical		induce					Colon tumors	MedicalFinding				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_22_2_315_s_27	11181454	Colon tumors induced by DMH contain Ki- ras mutations but lack genetic changes in  p53 ( 26), whereas those induced by IQ lack mutations in Ki- ras and  p53 genes, and have few microsatellite or  Apc mutations ( 27).	transcription
72783	2	336291	7	NULL	NULL	0	NULL	Colon tumors	MedicalFinding		contain					Ki- ras mutations	Process				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_22_2_315_s_27	11181454	Colon tumors induced by DMH contain Ki- ras mutations but lack genetic changes in  p53 ( 26), whereas those induced by IQ lack mutations in Ki- ras and  p53 genes, and have few microsatellite or  Apc mutations ( 27).	transcription
72784	3	336291	7	NULL	NULL	0	NULL	statement 2	Process		lack					p53	GP	genetic changes in			NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_22_2_315_s_27	11181454	Colon tumors induced by DMH contain Ki- ras mutations but lack genetic changes in  p53 ( 26), whereas those induced by IQ lack mutations in Ki- ras and  p53 genes, and have few microsatellite or  Apc mutations ( 27).	transcription
72785	4	336291	7	NULL	NULL	0	NULL	IQ	Chemical		induce					Colon tumors	MedicalFinding				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_22_2_315_s_27	11181454	Colon tumors induced by DMH contain Ki- ras mutations but lack genetic changes in  p53 ( 26), whereas those induced by IQ lack mutations in Ki- ras and  p53 genes, and have few microsatellite or  Apc mutations ( 27).	transcription
72786	5	336291	7	NULL	NULL	NULL	NULL	statement 4	Process		lack					Ki-ras gene	GP	mutations in			NULL		NULL	NULL	NULL	NULL	gw60_carcinogenesis_22_2_315_s_27	11181454	Colon tumors induced by DMH contain Ki- ras mutations but lack genetic changes in  p53 ( 26), whereas those induced by IQ lack mutations in Ki- ras and  p53 genes, and have few microsatellite or  Apc mutations ( 27).	transcription
72787	6	336291	7	NULL	NULL	0	NULL	statement 4	Process		lack					p53 gene	GP	mutations in			NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_22_2_315_s_27	11181454	Colon tumors induced by DMH contain Ki- ras mutations but lack genetic changes in  p53 ( 26), whereas those induced by IQ lack mutations in Ki- ras and  p53 genes, and have few microsatellite or  Apc mutations ( 27).	transcription
72788	7	336291	7	NULL	NULL	0	NULL	statement 4	Process		contain					microsatellite mutations	Process				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_22_2_315_s_27	11181454	Colon tumors induced by DMH contain Ki- ras mutations but lack genetic changes in  p53 ( 26), whereas those induced by IQ lack mutations in Ki- ras and  p53 genes, and have few microsatellite or  Apc mutations ( 27).	transcription
72789	8	336291	7	NULL	NULL	0	NULL	statement 4	Process		contain					Apc mutations	Process				NULL		0	NULL	NULL	NULL	gw60_carcinogenesis_22_2_315_s_27	11181454	Colon tumors induced by DMH contain Ki- ras mutations but lack genetic changes in  p53 ( 26), whereas those induced by IQ lack mutations in Ki- ras and  p53 genes, and have few microsatellite or  Apc mutations ( 27).	transcription
72790	1	336292	7	NULL	NULL	0	NULL	cells	Cell		progressed to					Cell cycle	Process				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_7_2844_s_317	12857869	Our present results support that in cell lines with normal  APC and p53 products, such as epidermal keratinocytes analyzed here, a tight  regulation of cytoplasmic beta-catenin (nonassociated to adhesion complexes)  during G2 to M transition is required to allow the correct progression of  cells into the cell cycle.	transcription
72791	2	336292	7	NULL	NULL	NULL	NULL	beta-catenin	GP	tight regulation of;;cytoplasmic	required for					statement 1	Process	correct progression of			NULL	epidermal keratinocytes  with normal APC products	NULL	NULL	NULL	NULL	gw60_molbiolcell_14_7_2844_s_317	12857869	Our present results support that in cell lines with normal  APC and p53 products, such as epidermal keratinocytes analyzed here, a tight  regulation of cytoplasmic beta-catenin (nonassociated to adhesion complexes)  during G2 to M transition is required to allow the correct progression of  cells into the cell cycle.	transcription
72792	3	336292	7	NULL	NULL	NULL	NULL	beta-catenin	GP	tight regulation of;;cytoplasmic	required for					statement 1	Process	correct progression of			NULL	epidermal keratinocytes  with normal p53 products	NULL	NULL	NULL	NULL	gw60_molbiolcell_14_7_2844_s_317	12857869	Our present results support that in cell lines with normal  APC and p53 products, such as epidermal keratinocytes analyzed here, a tight  regulation of cytoplasmic beta-catenin (nonassociated to adhesion complexes)  during G2 to M transition is required to allow the correct progression of  cells into the cell cycle.	transcription
72793	4	336292	7	NULL	NULL	0	NULL	G2	Process		transition to					M	Process				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_7_2844_s_317	12857869	Our present results support that in cell lines with normal  APC and p53 products, such as epidermal keratinocytes analyzed here, a tight  regulation of cytoplasmic beta-catenin (nonassociated to adhesion complexes)  during G2 to M transition is required to allow the correct progression of  cells into the cell cycle.	transcription
72794	5	336292	7	NULL	NULL	0	NULL	statement 2	Process		occur during					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_7_2844_s_317	12857869	Our present results support that in cell lines with normal  APC and p53 products, such as epidermal keratinocytes analyzed here, a tight  regulation of cytoplasmic beta-catenin (nonassociated to adhesion complexes)  during G2 to M transition is required to allow the correct progression of  cells into the cell cycle.	transcription
72795	6	336292	7	NULL	NULL	0	NULL	statement 3	Process		occur during					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_7_2844_s_317	12857869	Our present results support that in cell lines with normal  APC and p53 products, such as epidermal keratinocytes analyzed here, a tight  regulation of cytoplasmic beta-catenin (nonassociated to adhesion complexes)  during G2 to M transition is required to allow the correct progression of  cells into the cell cycle.	transcription
72796	7	336292	7	NULL	NULL	0	NULL	beta-catenin	GP		nonassociated to					adhesion complex	GP				NULL		0	NULL	NULL	NULL	gw60_molbiolcell_14_7_2844_s_317	12857869	Our present results support that in cell lines with normal  APC and p53 products, such as epidermal keratinocytes analyzed here, a tight  regulation of cytoplasmic beta-catenin (nonassociated to adhesion complexes)  during G2 to M transition is required to allow the correct progression of  cells into the cell cycle.	transcription
72797	1	336293	7	NULL	NULL	0	NULL	MNNG	Chemical		cause					colon cancer	MedicalFinding				NULL	animals	0	NULL	NULL	NULL	gw60_jbiolchem_272_49_30619_s_3	9388195	In this study we treated  the HCT-116 colon cancer cell line with alkylating agents including  N-methyl- N -nitro- N-nitrosoguanidine (MNNG),which is known to cause colon cancer in animals, and examined the expression of both  APC and  p53 genes.	transcription
72798	2	336293	7	NULL	NULL	0	NULL	MNNG	Chemical		is					N-methyl- N -nitro- N-nitrosoguanidine	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_49_30619_s_3	9388195	In this study we treated  the HCT-116 colon cancer cell line with alkylating agents including  N-methyl- N -nitro- N-nitrosoguanidine (MNNG),which is known to cause colon cancer in animals, and examined the expression of both  APC and  p53 genes.	transcription
72799	3	336293	7	NULL	NULL	0	NULL	MNNG	Chemical		is a type of					alkylating agent	Chemical				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_272_49_30619_s_3	9388195	In this study we treated  the HCT-116 colon cancer cell line with alkylating agents including  N-methyl- N -nitro- N-nitrosoguanidine (MNNG),which is known to cause colon cancer in animals, and examined the expression of both  APC and  p53 genes.	transcription
72803	1	336295	7	NULL	NULL	0	NULL	K-ras	GP	mutation in	increased in					Dukes' C tumors	MedicalFinding				NULL		0	NULL	NULL	NULL	gw60_pnas_99_14_9433_s_125	12093899	Interestingly, analysis of the relative contribution of APC, K-ras, and p53 to the overall mutation burden in early and advanced tumors demonstrated a statistically significant increase in the K-ras mutation frequency in Dukes' C tumors (Fig.  4 B), suggesting that altered K-ras function is an important determinant of tumor progression.	transcription
72804	2	336295	7	NULL	NULL	0	NULL	K-ras	GP	altered function of	determinant of		important			tumor progression	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_99_14_9433_s_125	12093899	Interestingly, analysis of the relative contribution of APC, K-ras, and p53 to the overall mutation burden in early and advanced tumors demonstrated a statistically significant increase in the K-ras mutation frequency in Dukes' C tumors (Fig.  4 B), suggesting that altered K-ras function is an important determinant of tumor progression.	transcription
72805	1	336296	7	NULL	NULL	0	NULL	Mdm2	GP		catalyze					Mdm2	GP	ubiquitination of			NULL		0	NULL	NULL	NULL	gw60_pnas_96_20_11364_s_17	10500182	Other E3s include Mdm2, which catalyzes both its own ubiquitination and that of p53 ( 6); the anaphase-promoting complex (APC); and other F box and cullin-containing complexes whose substrates include Sic1p, G1 cyclins, IkappaB, and beta-catenin ( 7).	transcription
72806	2	336296	7	NULL	NULL	0	NULL	Mdm2	GP		catalyze					p53	GP	ubiquitination of			NULL		0	NULL	NULL	NULL	gw60_pnas_96_20_11364_s_17	10500182	Other E3s include Mdm2, which catalyzes both its own ubiquitination and that of p53 ( 6); the anaphase-promoting complex (APC); and other F box and cullin-containing complexes whose substrates include Sic1p, G1 cyclins, IkappaB, and beta-catenin ( 7).	transcription
72807	3	336296	7	NULL	NULL	0	NULL	E3	GP		include					Mdm2	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_96_20_11364_s_17	10500182	Other E3s include Mdm2, which catalyzes both its own ubiquitination and that of p53 ( 6); the anaphase-promoting complex (APC); and other F box and cullin-containing complexes whose substrates include Sic1p, G1 cyclins, IkappaB, and beta-catenin ( 7).	transcription
72808	4	336296	7	NULL	NULL	0	NULL	E3	GP		include					APC	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_96_20_11364_s_17	10500182	Other E3s include Mdm2, which catalyzes both its own ubiquitination and that of p53 ( 6); the anaphase-promoting complex (APC); and other F box and cullin-containing complexes whose substrates include Sic1p, G1 cyclins, IkappaB, and beta-catenin ( 7).	transcription
72809	5	336296	7	NULL	NULL	0	NULL	E3	GP		include					F box	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_96_20_11364_s_17	10500182	Other E3s include Mdm2, which catalyzes both its own ubiquitination and that of p53 ( 6); the anaphase-promoting complex (APC); and other F box and cullin-containing complexes whose substrates include Sic1p, G1 cyclins, IkappaB, and beta-catenin ( 7).	transcription
72810	6	336296	7	NULL	NULL	0	NULL	E3	GP		include					cullin-containing complex	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_96_20_11364_s_17	10500182	Other E3s include Mdm2, which catalyzes both its own ubiquitination and that of p53 ( 6); the anaphase-promoting complex (APC); and other F box and cullin-containing complexes whose substrates include Sic1p, G1 cyclins, IkappaB, and beta-catenin ( 7).	transcription
72811	7	336296	7	NULL	NULL	0	NULL	APC	GP		is					anaphase-promoting complex	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_96_20_11364_s_17	10500182	Other E3s include Mdm2, which catalyzes both its own ubiquitination and that of p53 ( 6); the anaphase-promoting complex (APC); and other F box and cullin-containing complexes whose substrates include Sic1p, G1 cyclins, IkappaB, and beta-catenin ( 7).	transcription
72812	8	336296	7	NULL	NULL	0	NULL	cullin-containing complex	GP	substrate of	include					Sic1p	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_96_20_11364_s_17	10500182	Other E3s include Mdm2, which catalyzes both its own ubiquitination and that of p53 ( 6); the anaphase-promoting complex (APC); and other F box and cullin-containing complexes whose substrates include Sic1p, G1 cyclins, IkappaB, and beta-catenin ( 7).	transcription
72813	9	336296	7	NULL	NULL	0	NULL	cullin-containing complex	GP	substrate of	include					G1 cyclins	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_96_20_11364_s_17	10500182	Other E3s include Mdm2, which catalyzes both its own ubiquitination and that of p53 ( 6); the anaphase-promoting complex (APC); and other F box and cullin-containing complexes whose substrates include Sic1p, G1 cyclins, IkappaB, and beta-catenin ( 7).	transcription
72814	10	336296	7	NULL	NULL	0	NULL	cullin-containing complex	GP	substrate of	include					 IkappaB	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_96_20_11364_s_17	10500182	Other E3s include Mdm2, which catalyzes both its own ubiquitination and that of p53 ( 6); the anaphase-promoting complex (APC); and other F box and cullin-containing complexes whose substrates include Sic1p, G1 cyclins, IkappaB, and beta-catenin ( 7).	transcription
72815	11	336296	7	NULL	NULL	0	NULL	cullin-containing complex	GP	substrate of	include					beta-catenin	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_96_20_11364_s_17	10500182	Other E3s include Mdm2, which catalyzes both its own ubiquitination and that of p53 ( 6); the anaphase-promoting complex (APC); and other F box and cullin-containing complexes whose substrates include Sic1p, G1 cyclins, IkappaB, and beta-catenin ( 7).	transcription
72816	1	336297	7	NULL	NULL	0	NULL	APC	GP		induced by					quercetin	Chemical				NULL		0	NULL	NULL	NULL	gw70_clindiagnlabimmun_11_1_63_s_94	14715546	Furthermore, the six tumor suppressor genes adenomatosis polyposis coli ( APC), transforming growth factor beta receptor 11 ( TGFbetaR2), tumor suppressor protein p53 (p53), retinoblastoma 1 ( Rb), cyclin-dependent kinase inhbitor 1C (p57Kip2), and tuberous sclerosis 2 ( TSC-2) were induced by quercetin, whereas undetectable levels of these genes were expressed by control, untreated PC-3 cells.	transcription
72817	2	336297	7	NULL	NULL	0	NULL	TGFbetaR2	GP		induced by					quercetin	Chemical				NULL		0	NULL	NULL	NULL	gw70_clindiagnlabimmun_11_1_63_s_94	14715546	Furthermore, the six tumor suppressor genes adenomatosis polyposis coli ( APC), transforming growth factor beta receptor 11 ( TGFbetaR2), tumor suppressor protein p53 (p53), retinoblastoma 1 ( Rb), cyclin-dependent kinase inhbitor 1C (p57Kip2), and tuberous sclerosis 2 ( TSC-2) were induced by quercetin, whereas undetectable levels of these genes were expressed by control, untreated PC-3 cells.	transcription
72818	3	336297	7	NULL	NULL	0	NULL	p53	GP		induced by					quercetin	Chemical				NULL		0	NULL	NULL	NULL	gw70_clindiagnlabimmun_11_1_63_s_94	14715546	Furthermore, the six tumor suppressor genes adenomatosis polyposis coli ( APC), transforming growth factor beta receptor 11 ( TGFbetaR2), tumor suppressor protein p53 (p53), retinoblastoma 1 ( Rb), cyclin-dependent kinase inhbitor 1C (p57Kip2), and tuberous sclerosis 2 ( TSC-2) were induced by quercetin, whereas undetectable levels of these genes were expressed by control, untreated PC-3 cells.	transcription
72819	4	336297	7	NULL	NULL	0	NULL	Rb	GP		induced by					quercetin	Chemical				NULL		0	NULL	NULL	NULL	gw70_clindiagnlabimmun_11_1_63_s_94	14715546	Furthermore, the six tumor suppressor genes adenomatosis polyposis coli ( APC), transforming growth factor beta receptor 11 ( TGFbetaR2), tumor suppressor protein p53 (p53), retinoblastoma 1 ( Rb), cyclin-dependent kinase inhbitor 1C (p57Kip2), and tuberous sclerosis 2 ( TSC-2) were induced by quercetin, whereas undetectable levels of these genes were expressed by control, untreated PC-3 cells.	transcription
72820	5	336297	7	NULL	NULL	0	NULL	p57Kip2	GP		induced by					quercetin	Chemical				NULL		0	NULL	NULL	NULL	gw70_clindiagnlabimmun_11_1_63_s_94	14715546	Furthermore, the six tumor suppressor genes adenomatosis polyposis coli ( APC), transforming growth factor beta receptor 11 ( TGFbetaR2), tumor suppressor protein p53 (p53), retinoblastoma 1 ( Rb), cyclin-dependent kinase inhbitor 1C (p57Kip2), and tuberous sclerosis 2 ( TSC-2) were induced by quercetin, whereas undetectable levels of these genes were expressed by control, untreated PC-3 cells.	transcription
72821	6	336297	7	NULL	NULL	0	NULL	TSC-2	GP		induced by					quercetin	Chemical				NULL		0	NULL	NULL	NULL	gw70_clindiagnlabimmun_11_1_63_s_94	14715546	Furthermore, the six tumor suppressor genes adenomatosis polyposis coli ( APC), transforming growth factor beta receptor 11 ( TGFbetaR2), tumor suppressor protein p53 (p53), retinoblastoma 1 ( Rb), cyclin-dependent kinase inhbitor 1C (p57Kip2), and tuberous sclerosis 2 ( TSC-2) were induced by quercetin, whereas undetectable levels of these genes were expressed by control, untreated PC-3 cells.	transcription
72822	7	336297	7	NULL	NULL	0	NULL	APC	GP		is					adenomatosis polyposis coli	GP				NULL		0	NULL	NULL	NULL	gw70_clindiagnlabimmun_11_1_63_s_94	14715546	Furthermore, the six tumor suppressor genes adenomatosis polyposis coli ( APC), transforming growth factor beta receptor 11 ( TGFbetaR2), tumor suppressor protein p53 (p53), retinoblastoma 1 ( Rb), cyclin-dependent kinase inhbitor 1C (p57Kip2), and tuberous sclerosis 2 ( TSC-2) were induced by quercetin, whereas undetectable levels of these genes were expressed by control, untreated PC-3 cells.	transcription
72823	8	336297	7	NULL	NULL	0	NULL	APC	GP		is a type of					tumor suppressor genes	GP				NULL		0	NULL	NULL	NULL	gw70_clindiagnlabimmun_11_1_63_s_94	14715546	Furthermore, the six tumor suppressor genes adenomatosis polyposis coli ( APC), transforming growth factor beta receptor 11 ( TGFbetaR2), tumor suppressor protein p53 (p53), retinoblastoma 1 ( Rb), cyclin-dependent kinase inhbitor 1C (p57Kip2), and tuberous sclerosis 2 ( TSC-2) were induced by quercetin, whereas undetectable levels of these genes were expressed by control, untreated PC-3 cells.	transcription
72824	9	336297	7	NULL	NULL	0	NULL	TGFbetaR2	GP		is					transforming growth factor beta receptor 11	GP				NULL		0	NULL	NULL	NULL	gw70_clindiagnlabimmun_11_1_63_s_94	14715546	Furthermore, the six tumor suppressor genes adenomatosis polyposis coli ( APC), transforming growth factor beta receptor 11 ( TGFbetaR2), tumor suppressor protein p53 (p53), retinoblastoma 1 ( Rb), cyclin-dependent kinase inhbitor 1C (p57Kip2), and tuberous sclerosis 2 ( TSC-2) were induced by quercetin, whereas undetectable levels of these genes were expressed by control, untreated PC-3 cells.	transcription
72825	10	336297	7	NULL	NULL	NULL	NULL	TGFbetaR2	GP		is a type of					tumor suppressor genes	GP				NULL		NULL	NULL	NULL	NULL	gw70_clindiagnlabimmun_11_1_63_s_94	14715546	Furthermore, the six tumor suppressor genes adenomatosis polyposis coli ( APC), transforming growth factor beta receptor 11 ( TGFbetaR2), tumor suppressor protein p53 (p53), retinoblastoma 1 ( Rb), cyclin-dependent kinase inhbitor 1C (p57Kip2), and tuberous sclerosis 2 ( TSC-2) were induced by quercetin, whereas undetectable levels of these genes were expressed by control, untreated PC-3 cells.	transcription
72826	11	336297	7	NULL	NULL	0	NULL	p53	GP		is a type of					tumor suppressor protein	GP				NULL		0	NULL	NULL	NULL	gw70_clindiagnlabimmun_11_1_63_s_94	14715546	Furthermore, the six tumor suppressor genes adenomatosis polyposis coli ( APC), transforming growth factor beta receptor 11 ( TGFbetaR2), tumor suppressor protein p53 (p53), retinoblastoma 1 ( Rb), cyclin-dependent kinase inhbitor 1C (p57Kip2), and tuberous sclerosis 2 ( TSC-2) were induced by quercetin, whereas undetectable levels of these genes were expressed by control, untreated PC-3 cells.	transcription
72827	12	336297	7	NULL	NULL	0	NULL	Rb	GP		is 					retinoblastoma 1	GP				NULL		0	NULL	NULL	NULL	gw70_clindiagnlabimmun_11_1_63_s_94	14715546	Furthermore, the six tumor suppressor genes adenomatosis polyposis coli ( APC), transforming growth factor beta receptor 11 ( TGFbetaR2), tumor suppressor protein p53 (p53), retinoblastoma 1 ( Rb), cyclin-dependent kinase inhbitor 1C (p57Kip2), and tuberous sclerosis 2 ( TSC-2) were induced by quercetin, whereas undetectable levels of these genes were expressed by control, untreated PC-3 cells.	transcription
72828	13	336297	7	NULL	NULL	0	NULL	Rb	GP		is a type of					tumor suppressor genes	GP				NULL		0	NULL	NULL	NULL	gw70_clindiagnlabimmun_11_1_63_s_94	14715546	Furthermore, the six tumor suppressor genes adenomatosis polyposis coli ( APC), transforming growth factor beta receptor 11 ( TGFbetaR2), tumor suppressor protein p53 (p53), retinoblastoma 1 ( Rb), cyclin-dependent kinase inhbitor 1C (p57Kip2), and tuberous sclerosis 2 ( TSC-2) were induced by quercetin, whereas undetectable levels of these genes were expressed by control, untreated PC-3 cells.	transcription
72829	14	336297	7	NULL	NULL	NULL	NULL	p57Kip2	GP		is a type of					cyclin-dependent kinase inhbitor 1C	GP				NULL		NULL	NULL	NULL	NULL	gw70_clindiagnlabimmun_11_1_63_s_94	14715546	Furthermore, the six tumor suppressor genes adenomatosis polyposis coli ( APC), transforming growth factor beta receptor 11 ( TGFbetaR2), tumor suppressor protein p53 (p53), retinoblastoma 1 ( Rb), cyclin-dependent kinase inhbitor 1C (p57Kip2), and tuberous sclerosis 2 ( TSC-2) were induced by quercetin, whereas undetectable levels of these genes were expressed by control, untreated PC-3 cells.	transcription
72830	15	336297	7	NULL	NULL	NULL	NULL	p57Kip2	GP		is a type of					tumor suppressor genes	GP				NULL		NULL	NULL	NULL	NULL	gw70_clindiagnlabimmun_11_1_63_s_94	14715546	Furthermore, the six tumor suppressor genes adenomatosis polyposis coli ( APC), transforming growth factor beta receptor 11 ( TGFbetaR2), tumor suppressor protein p53 (p53), retinoblastoma 1 ( Rb), cyclin-dependent kinase inhbitor 1C (p57Kip2), and tuberous sclerosis 2 ( TSC-2) were induced by quercetin, whereas undetectable levels of these genes were expressed by control, untreated PC-3 cells.	transcription
72831	16	336297	7	NULL	NULL	0	NULL	TSC-2	GP		is					tuberous sclerosis 2	GP				NULL		0	NULL	NULL	NULL	gw70_clindiagnlabimmun_11_1_63_s_94	14715546	Furthermore, the six tumor suppressor genes adenomatosis polyposis coli ( APC), transforming growth factor beta receptor 11 ( TGFbetaR2), tumor suppressor protein p53 (p53), retinoblastoma 1 ( Rb), cyclin-dependent kinase inhbitor 1C (p57Kip2), and tuberous sclerosis 2 ( TSC-2) were induced by quercetin, whereas undetectable levels of these genes were expressed by control, untreated PC-3 cells.	transcription
72832	17	336297	7	NULL	NULL	0	NULL	TSC-2	GP		is a type of					tumor suppressor genes	GP				NULL		0	NULL	NULL	NULL	gw70_clindiagnlabimmun_11_1_63_s_94	14715546	Furthermore, the six tumor suppressor genes adenomatosis polyposis coli ( APC), transforming growth factor beta receptor 11 ( TGFbetaR2), tumor suppressor protein p53 (p53), retinoblastoma 1 ( Rb), cyclin-dependent kinase inhbitor 1C (p57Kip2), and tuberous sclerosis 2 ( TSC-2) were induced by quercetin, whereas undetectable levels of these genes were expressed by control, untreated PC-3 cells.	transcription
72833	1	336298	7	NULL	NULL	0	NULL	IkappaB 	GP		is a type of					transcriptional regulator	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_6_2999_s_11	15814838	These motors transport mRNAs for cell fate and polarity determinations (reviewed in Saxton, 2001 ), transcriptional regulators, such as the NF kappa B inhibitor IkappaB (Crepieux  et al., 1997 ), the tumor suppressor protein p53 (Giannakakou  et al., 2000 ; Giannakakou  et al., 2002 ), the developmental factors beta-catenin or adenomatous poliposis coli protein (APC, reviewed in Bienz, 2002 ), the apoptosis effector bim (Puthalakath  et al., 1999 ), and stress-related signaling kinases of the ERK and JNK families (reviewed in Verhey and Rapoport, 2001 ).	transcription
72834	2	336298	7	NULL	NULL	0	NULL	IkappaB	GP		inhibit					NF kappa B	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_6_2999_s_11	15814838	These motors transport mRNAs for cell fate and polarity determinations (reviewed in Saxton, 2001 ), transcriptional regulators, such as the NF kappa B inhibitor IkappaB (Crepieux  et al., 1997 ), the tumor suppressor protein p53 (Giannakakou  et al., 2000 ; Giannakakou  et al., 2002 ), the developmental factors beta-catenin or adenomatous poliposis coli protein (APC, reviewed in Bienz, 2002 ), the apoptosis effector bim (Puthalakath  et al., 1999 ), and stress-related signaling kinases of the ERK and JNK families (reviewed in Verhey and Rapoport, 2001 ).	transcription
72835	3	336298	7	NULL	NULL	0	NULL	p53	GP		is a type of					tumor suppressor protein	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_6_2999_s_11	15814838	These motors transport mRNAs for cell fate and polarity determinations (reviewed in Saxton, 2001 ), transcriptional regulators, such as the NF kappa B inhibitor IkappaB (Crepieux  et al., 1997 ), the tumor suppressor protein p53 (Giannakakou  et al., 2000 ; Giannakakou  et al., 2002 ), the developmental factors beta-catenin or adenomatous poliposis coli protein (APC, reviewed in Bienz, 2002 ), the apoptosis effector bim (Puthalakath  et al., 1999 ), and stress-related signaling kinases of the ERK and JNK families (reviewed in Verhey and Rapoport, 2001 ).	transcription
72836	4	336298	7	NULL	NULL	0	NULL	p53	GP		is a type of					transcriptional regulator	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_6_2999_s_11	15814838	These motors transport mRNAs for cell fate and polarity determinations (reviewed in Saxton, 2001 ), transcriptional regulators, such as the NF kappa B inhibitor IkappaB (Crepieux  et al., 1997 ), the tumor suppressor protein p53 (Giannakakou  et al., 2000 ; Giannakakou  et al., 2002 ), the developmental factors beta-catenin or adenomatous poliposis coli protein (APC, reviewed in Bienz, 2002 ), the apoptosis effector bim (Puthalakath  et al., 1999 ), and stress-related signaling kinases of the ERK and JNK families (reviewed in Verhey and Rapoport, 2001 ).	transcription
72837	5	336298	7	NULL	NULL	0	NULL	 beta-catenin	GP		is a type of					developmental factor	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_6_2999_s_11	15814838	These motors transport mRNAs for cell fate and polarity determinations (reviewed in Saxton, 2001 ), transcriptional regulators, such as the NF kappa B inhibitor IkappaB (Crepieux  et al., 1997 ), the tumor suppressor protein p53 (Giannakakou  et al., 2000 ; Giannakakou  et al., 2002 ), the developmental factors beta-catenin or adenomatous poliposis coli protein (APC, reviewed in Bienz, 2002 ), the apoptosis effector bim (Puthalakath  et al., 1999 ), and stress-related signaling kinases of the ERK and JNK families (reviewed in Verhey and Rapoport, 2001 ).	transcription
72838	6	336298	7	NULL	NULL	0	NULL	APC	GP		is a type of					developmental factor	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_6_2999_s_11	15814838	These motors transport mRNAs for cell fate and polarity determinations (reviewed in Saxton, 2001 ), transcriptional regulators, such as the NF kappa B inhibitor IkappaB (Crepieux  et al., 1997 ), the tumor suppressor protein p53 (Giannakakou  et al., 2000 ; Giannakakou  et al., 2002 ), the developmental factors beta-catenin or adenomatous poliposis coli protein (APC, reviewed in Bienz, 2002 ), the apoptosis effector bim (Puthalakath  et al., 1999 ), and stress-related signaling kinases of the ERK and JNK families (reviewed in Verhey and Rapoport, 2001 ).	transcription
72839	7	336298	7	NULL	NULL	0	NULL	beta-catenin	GP		is a type of					transcriptional regulator	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_6_2999_s_11	15814838	These motors transport mRNAs for cell fate and polarity determinations (reviewed in Saxton, 2001 ), transcriptional regulators, such as the NF kappa B inhibitor IkappaB (Crepieux  et al., 1997 ), the tumor suppressor protein p53 (Giannakakou  et al., 2000 ; Giannakakou  et al., 2002 ), the developmental factors beta-catenin or adenomatous poliposis coli protein (APC, reviewed in Bienz, 2002 ), the apoptosis effector bim (Puthalakath  et al., 1999 ), and stress-related signaling kinases of the ERK and JNK families (reviewed in Verhey and Rapoport, 2001 ).	transcription
72840	8	336298	7	NULL	NULL	0	NULL	APC	GP		is a type of					adenomatous poliposis coli protein	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_6_2999_s_11	15814838	These motors transport mRNAs for cell fate and polarity determinations (reviewed in Saxton, 2001 ), transcriptional regulators, such as the NF kappa B inhibitor IkappaB (Crepieux  et al., 1997 ), the tumor suppressor protein p53 (Giannakakou  et al., 2000 ; Giannakakou  et al., 2002 ), the developmental factors beta-catenin or adenomatous poliposis coli protein (APC, reviewed in Bienz, 2002 ), the apoptosis effector bim (Puthalakath  et al., 1999 ), and stress-related signaling kinases of the ERK and JNK families (reviewed in Verhey and Rapoport, 2001 ).	transcription
72841	9	336298	7	NULL	NULL	NULL	NULL	APC	GP		is a type of					transcriptional regulator	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_6_2999_s_11	15814838	These motors transport mRNAs for cell fate and polarity determinations (reviewed in Saxton, 2001 ), transcriptional regulators, such as the NF kappa B inhibitor IkappaB (Crepieux  et al., 1997 ), the tumor suppressor protein p53 (Giannakakou  et al., 2000 ; Giannakakou  et al., 2002 ), the developmental factors beta-catenin or adenomatous poliposis coli protein (APC, reviewed in Bienz, 2002 ), the apoptosis effector bim (Puthalakath  et al., 1999 ), and stress-related signaling kinases of the ERK and JNK families (reviewed in Verhey and Rapoport, 2001 ).	transcription
72842	10	336298	7	NULL	NULL	NULL	NULL	bim	GP		is a type of					apoptosis effector	GP				NULL		NULL	NULL	NULL	NULL	gw70_molbiolcell_16_6_2999_s_11	15814838	These motors transport mRNAs for cell fate and polarity determinations (reviewed in Saxton, 2001 ), transcriptional regulators, such as the NF kappa B inhibitor IkappaB (Crepieux  et al., 1997 ), the tumor suppressor protein p53 (Giannakakou  et al., 2000 ; Giannakakou  et al., 2002 ), the developmental factors beta-catenin or adenomatous poliposis coli protein (APC, reviewed in Bienz, 2002 ), the apoptosis effector bim (Puthalakath  et al., 1999 ), and stress-related signaling kinases of the ERK and JNK families (reviewed in Verhey and Rapoport, 2001 ).	transcription
72843	11	336298	7	NULL	NULL	0	NULL	ERK family	GP		is a type of					stress-related signaling kinases	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_6_2999_s_11	15814838	These motors transport mRNAs for cell fate and polarity determinations (reviewed in Saxton, 2001 ), transcriptional regulators, such as the NF kappa B inhibitor IkappaB (Crepieux  et al., 1997 ), the tumor suppressor protein p53 (Giannakakou  et al., 2000 ; Giannakakou  et al., 2002 ), the developmental factors beta-catenin or adenomatous poliposis coli protein (APC, reviewed in Bienz, 2002 ), the apoptosis effector bim (Puthalakath  et al., 1999 ), and stress-related signaling kinases of the ERK and JNK families (reviewed in Verhey and Rapoport, 2001 ).	transcription
72844	12	336298	7	NULL	NULL	0	NULL	JNK family	GP		is a type of					stress-related signaling kinases	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_6_2999_s_11	15814838	These motors transport mRNAs for cell fate and polarity determinations (reviewed in Saxton, 2001 ), transcriptional regulators, such as the NF kappa B inhibitor IkappaB (Crepieux  et al., 1997 ), the tumor suppressor protein p53 (Giannakakou  et al., 2000 ; Giannakakou  et al., 2002 ), the developmental factors beta-catenin or adenomatous poliposis coli protein (APC, reviewed in Bienz, 2002 ), the apoptosis effector bim (Puthalakath  et al., 1999 ), and stress-related signaling kinases of the ERK and JNK families (reviewed in Verhey and Rapoport, 2001 ).	transcription
72845	13	336298	7	NULL	NULL	0	NULL	bim	GP		is a type of					transcriptional regulator	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_6_2999_s_11	15814838	These motors transport mRNAs for cell fate and polarity determinations (reviewed in Saxton, 2001 ), transcriptional regulators, such as the NF kappa B inhibitor IkappaB (Crepieux  et al., 1997 ), the tumor suppressor protein p53 (Giannakakou  et al., 2000 ; Giannakakou  et al., 2002 ), the developmental factors beta-catenin or adenomatous poliposis coli protein (APC, reviewed in Bienz, 2002 ), the apoptosis effector bim (Puthalakath  et al., 1999 ), and stress-related signaling kinases of the ERK and JNK families (reviewed in Verhey and Rapoport, 2001 ).	transcription
72846	14	336298	7	NULL	NULL	0	NULL	ERK family	GP		is a type of					transcriptional regulator	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_6_2999_s_11	15814838	These motors transport mRNAs for cell fate and polarity determinations (reviewed in Saxton, 2001 ), transcriptional regulators, such as the NF kappa B inhibitor IkappaB (Crepieux  et al., 1997 ), the tumor suppressor protein p53 (Giannakakou  et al., 2000 ; Giannakakou  et al., 2002 ), the developmental factors beta-catenin or adenomatous poliposis coli protein (APC, reviewed in Bienz, 2002 ), the apoptosis effector bim (Puthalakath  et al., 1999 ), and stress-related signaling kinases of the ERK and JNK families (reviewed in Verhey and Rapoport, 2001 ).	transcription
72847	15	336298	7	NULL	NULL	0	NULL	JNK family	GP		is a type of					transcriptional regulator	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_16_6_2999_s_11	15814838	These motors transport mRNAs for cell fate and polarity determinations (reviewed in Saxton, 2001 ), transcriptional regulators, such as the NF kappa B inhibitor IkappaB (Crepieux  et al., 1997 ), the tumor suppressor protein p53 (Giannakakou  et al., 2000 ; Giannakakou  et al., 2002 ), the developmental factors beta-catenin or adenomatous poliposis coli protein (APC, reviewed in Bienz, 2002 ), the apoptosis effector bim (Puthalakath  et al., 1999 ), and stress-related signaling kinases of the ERK and JNK families (reviewed in Verhey and Rapoport, 2001 ).	transcription
72848	1	336299	7	NULL	NULL	0	NULL	 proliferation	Process	increase in	associated with					 beta-cat	GP				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_5_1619_s_373	12414510	14, 20, 62  This beta-cat-associated increase in proliferation is tightly controlled by the following mechanisms: 1) nuclear sequestration 10, 11  and cytoplasmic degradation of beta-cat by APC; 2- 9  2) activation of p53, that accumulates in response to beta-cat signaling and triggers a cell growth arrest; 15- 17  and 3) p27KIP-dependent cell-cycle arrest that results from the interplay between activation of nuclear beta-cat transcriptional targets (eg, myc 76 ) and E-cad.	transcription
72849	2	336299	7	NULL	NULL	0	NULL	APC	GP		sequesters		nuclear			beta-cat	GP				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_5_1619_s_373	12414510	14, 20, 62  This beta-cat-associated increase in proliferation is tightly controlled by the following mechanisms: 1) nuclear sequestration 10, 11  and cytoplasmic degradation of beta-cat by APC; 2- 9  2) activation of p53, that accumulates in response to beta-cat signaling and triggers a cell growth arrest; 15- 17  and 3) p27KIP-dependent cell-cycle arrest that results from the interplay between activation of nuclear beta-cat transcriptional targets (eg, myc 76 ) and E-cad.	transcription
72850	3	336299	7	NULL	NULL	0	NULL	APC	GP		degrades					beta-cat	GP	cytoplasmic			NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_5_1619_s_373	12414510	14, 20, 62  This beta-cat-associated increase in proliferation is tightly controlled by the following mechanisms: 1) nuclear sequestration 10, 11  and cytoplasmic degradation of beta-cat by APC; 2- 9  2) activation of p53, that accumulates in response to beta-cat signaling and triggers a cell growth arrest; 15- 17  and 3) p27KIP-dependent cell-cycle arrest that results from the interplay between activation of nuclear beta-cat transcriptional targets (eg, myc 76 ) and E-cad.	transcription
72851	4	336299	7	NULL	NULL	0	NULL	p53	GP	activation of	accumulate					beta-cat signaling	Process	in response to			NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_5_1619_s_373	12414510	14, 20, 62  This beta-cat-associated increase in proliferation is tightly controlled by the following mechanisms: 1) nuclear sequestration 10, 11  and cytoplasmic degradation of beta-cat by APC; 2- 9  2) activation of p53, that accumulates in response to beta-cat signaling and triggers a cell growth arrest; 15- 17  and 3) p27KIP-dependent cell-cycle arrest that results from the interplay between activation of nuclear beta-cat transcriptional targets (eg, myc 76 ) and E-cad.	transcription
72852	5	336299	7	NULL	NULL	NULL	NULL	statement 4	Process		triggers					cell growth arrest	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_5_1619_s_373	12414510	14, 20, 62  This beta-cat-associated increase in proliferation is tightly controlled by the following mechanisms: 1) nuclear sequestration 10, 11  and cytoplasmic degradation of beta-cat by APC; 2- 9  2) activation of p53, that accumulates in response to beta-cat signaling and triggers a cell growth arrest; 15- 17  and 3) p27KIP-dependent cell-cycle arrest that results from the interplay between activation of nuclear beta-cat transcriptional targets (eg, myc 76 ) and E-cad.	transcription
72853	6	336299	7	NULL	NULL	0	NULL	cell-cycle arrest	Process		depends on					 p27KIP	GP				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_5_1619_s_373	12414510	14, 20, 62  This beta-cat-associated increase in proliferation is tightly controlled by the following mechanisms: 1) nuclear sequestration 10, 11  and cytoplasmic degradation of beta-cat by APC; 2- 9  2) activation of p53, that accumulates in response to beta-cat signaling and triggers a cell growth arrest; 15- 17  and 3) p27KIP-dependent cell-cycle arrest that results from the interplay between activation of nuclear beta-cat transcriptional targets (eg, myc 76 ) and E-cad.	transcription
72854	7	336299	7	NULL	NULL	NULL	NULL	beta-cat transcriptional targets 	GP	activation of;;nuclear	interplay with					E-cad	GP				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_5_1619_s_373	12414510	14, 20, 62  This beta-cat-associated increase in proliferation is tightly controlled by the following mechanisms: 1) nuclear sequestration 10, 11  and cytoplasmic degradation of beta-cat by APC; 2- 9  2) activation of p53, that accumulates in response to beta-cat signaling and triggers a cell growth arrest; 15- 17  and 3) p27KIP-dependent cell-cycle arrest that results from the interplay between activation of nuclear beta-cat transcriptional targets (eg, myc 76 ) and E-cad.	transcription
72855	8	336299	7	NULL	NULL	NULL	NULL	statement 6	Process		result from					statement 7	Process				NULL		NULL	NULL	NULL	NULL	gw60_amjpathol_161_5_1619_s_373	12414510	14, 20, 62  This beta-cat-associated increase in proliferation is tightly controlled by the following mechanisms: 1) nuclear sequestration 10, 11  and cytoplasmic degradation of beta-cat by APC; 2- 9  2) activation of p53, that accumulates in response to beta-cat signaling and triggers a cell growth arrest; 15- 17  and 3) p27KIP-dependent cell-cycle arrest that results from the interplay between activation of nuclear beta-cat transcriptional targets (eg, myc 76 ) and E-cad.	transcription
72856	9	336299	7	NULL	NULL	0	NULL	statement 1	Process		controlled by		tightly			statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_5_1619_s_373	12414510	14, 20, 62  This beta-cat-associated increase in proliferation is tightly controlled by the following mechanisms: 1) nuclear sequestration 10, 11  and cytoplasmic degradation of beta-cat by APC; 2- 9  2) activation of p53, that accumulates in response to beta-cat signaling and triggers a cell growth arrest; 15- 17  and 3) p27KIP-dependent cell-cycle arrest that results from the interplay between activation of nuclear beta-cat transcriptional targets (eg, myc 76 ) and E-cad.	transcription
72857	10	336299	7	NULL	NULL	0	NULL	statement 1	Process		controlled by		tightly			statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_5_1619_s_373	12414510	14, 20, 62  This beta-cat-associated increase in proliferation is tightly controlled by the following mechanisms: 1) nuclear sequestration 10, 11  and cytoplasmic degradation of beta-cat by APC; 2- 9  2) activation of p53, that accumulates in response to beta-cat signaling and triggers a cell growth arrest; 15- 17  and 3) p27KIP-dependent cell-cycle arrest that results from the interplay between activation of nuclear beta-cat transcriptional targets (eg, myc 76 ) and E-cad.	transcription
72858	11	336299	7	NULL	NULL	0	NULL	statement 1	Process		controlled by		tightly			statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_5_1619_s_373	12414510	14, 20, 62  This beta-cat-associated increase in proliferation is tightly controlled by the following mechanisms: 1) nuclear sequestration 10, 11  and cytoplasmic degradation of beta-cat by APC; 2- 9  2) activation of p53, that accumulates in response to beta-cat signaling and triggers a cell growth arrest; 15- 17  and 3) p27KIP-dependent cell-cycle arrest that results from the interplay between activation of nuclear beta-cat transcriptional targets (eg, myc 76 ) and E-cad.	transcription
72859	12	336299	7	NULL	NULL	0	NULL	statement 1	Process		controlled by		tightly			statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_5_1619_s_373	12414510	14, 20, 62  This beta-cat-associated increase in proliferation is tightly controlled by the following mechanisms: 1) nuclear sequestration 10, 11  and cytoplasmic degradation of beta-cat by APC; 2- 9  2) activation of p53, that accumulates in response to beta-cat signaling and triggers a cell growth arrest; 15- 17  and 3) p27KIP-dependent cell-cycle arrest that results from the interplay between activation of nuclear beta-cat transcriptional targets (eg, myc 76 ) and E-cad.	transcription
72860	13	336299	7	NULL	NULL	0	NULL	statement 1	Process		controlled by		tightly			statement 8	Process				NULL		0	NULL	NULL	NULL	gw60_amjpathol_161_5_1619_s_373	12414510	14, 20, 62  This beta-cat-associated increase in proliferation is tightly controlled by the following mechanisms: 1) nuclear sequestration 10, 11  and cytoplasmic degradation of beta-cat by APC; 2- 9  2) activation of p53, that accumulates in response to beta-cat signaling and triggers a cell growth arrest; 15- 17  and 3) p27KIP-dependent cell-cycle arrest that results from the interplay between activation of nuclear beta-cat transcriptional targets (eg, myc 76 ) and E-cad.	transcription
72861	1	336300	7	NULL	NULL	0	NULL	 TACC	GP		regulate					spindle structure	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_99_24_15440_s_193	12422018	It would not be surprising if future studies revealed an effect of p53 on the ability of Aur-A to associate with or regulate other interacting proteins, including the APC/C activator cdc20 ( 23), the translational regulator CPEB ( 24), the kinesin-like motor Eg5 ( 25), the transforming protein TACC that can regulate spindle structure ( 26), TPX2, which is required for targeting Aur-A to spindles ( 27), a newly identified protein called AIP that can promote Aur-A destruction ( 28), or others yet to be discovered.	transcription
72862	2	336300	7	NULL	NULL	0	NULL	TACC	GP		is a type of					transforming protein	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_99_24_15440_s_193	12422018	It would not be surprising if future studies revealed an effect of p53 on the ability of Aur-A to associate with or regulate other interacting proteins, including the APC/C activator cdc20 ( 23), the translational regulator CPEB ( 24), the kinesin-like motor Eg5 ( 25), the transforming protein TACC that can regulate spindle structure ( 26), TPX2, which is required for targeting Aur-A to spindles ( 27), a newly identified protein called AIP that can promote Aur-A destruction ( 28), or others yet to be discovered.	transcription
72863	3	336300	7	NULL	NULL	0	NULL	AurA	GP		targeted to					spindles	Chromosome				NULL		0	NULL	NULL	NULL	gw60_pnas_99_24_15440_s_193	12422018	It would not be surprising if future studies revealed an effect of p53 on the ability of Aur-A to associate with or regulate other interacting proteins, including the APC/C activator cdc20 ( 23), the translational regulator CPEB ( 24), the kinesin-like motor Eg5 ( 25), the transforming protein TACC that can regulate spindle structure ( 26), TPX2, which is required for targeting Aur-A to spindles ( 27), a newly identified protein called AIP that can promote Aur-A destruction ( 28), or others yet to be discovered.	transcription
72864	4	336300	7	NULL	NULL	0	NULL	TPX2	GP		is required for					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_99_24_15440_s_193	12422018	It would not be surprising if future studies revealed an effect of p53 on the ability of Aur-A to associate with or regulate other interacting proteins, including the APC/C activator cdc20 ( 23), the translational regulator CPEB ( 24), the kinesin-like motor Eg5 ( 25), the transforming protein TACC that can regulate spindle structure ( 26), TPX2, which is required for targeting Aur-A to spindles ( 27), a newly identified protein called AIP that can promote Aur-A destruction ( 28), or others yet to be discovered.	transcription
72865	5	336300	7	NULL	NULL	0	NULL	AIP	GP		promote					Aur-A	GP	destruction of			NULL		0	NULL	NULL	NULL	gw60_pnas_99_24_15440_s_193	12422018	It would not be surprising if future studies revealed an effect of p53 on the ability of Aur-A to associate with or regulate other interacting proteins, including the APC/C activator cdc20 ( 23), the translational regulator CPEB ( 24), the kinesin-like motor Eg5 ( 25), the transforming protein TACC that can regulate spindle structure ( 26), TPX2, which is required for targeting Aur-A to spindles ( 27), a newly identified protein called AIP that can promote Aur-A destruction ( 28), or others yet to be discovered.	transcription
72869	1	336301	7	NULL	NULL	NULL	NULL	reactions	Process		contains					p53	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_169	14612423	The addition of consensus site DNA to reactions containing p53, p300, and acetyl-coenzyme A (CoA) stimulates p53 acetylation ( ).	transcription
72870	2	336301	7	NULL	NULL	0	NULL	reactions	Process		contains					p300	GP				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_169	14612423	The addition of consensus site DNA to reactions containing p53, p300, and acetyl-coenzyme A (CoA) stimulates p53 acetylation ( ).	transcription
72871	3	336301	7	NULL	NULL	0	NULL	reactions	Process		contains					CoA	Chemical				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_169	14612423	The addition of consensus site DNA to reactions containing p53, p300, and acetyl-coenzyme A (CoA) stimulates p53 acetylation ( ).	transcription
72872	4	336301	7	NULL	NULL	0	NULL	CoA	Chemical		is					acetyl-coenzyme A	Chemical				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_169	14612423	The addition of consensus site DNA to reactions containing p53, p300, and acetyl-coenzyme A (CoA) stimulates p53 acetylation ( ).	transcription
72873	5	336301	7	NULL	NULL	0	NULL	statement 1	Process		stimulate					p53	GP	acetylation of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_169	14612423	The addition of consensus site DNA to reactions containing p53, p300, and acetyl-coenzyme A (CoA) stimulates p53 acetylation ( ).	transcription
72874	6	336301	7	NULL	NULL	0	NULL	statement 1	Process		stimulate					p300	GP	acetylation of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_169	14612423	The addition of consensus site DNA to reactions containing p53, p300, and acetyl-coenzyme A (CoA) stimulates p53 acetylation ( ).	transcription
72877	7	336301	7	NULL	NULL	0	NULL	statement 1	Process		stimulate					CoA	Chemical	acetylation of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_169	14612423	The addition of consensus site DNA to reactions containing p53, p300, and acetyl-coenzyme A (CoA) stimulates p53 acetylation ( ).	transcription
72885	1	336302	7	NULL	NULL	0	NULL	 Sirt1	GP	human	homologous to					Sir2a	GP	yeast			NULL		0	NULL	NULL	NULL	gw70_annurevpharmacol_45_0_269_s_168	15822178	The human homologue of yeast Sir2a, Sirt1,  inhibits p53 by removing the acetyl group from Lys382 in the C-terminal tail of p53  ( 85).	transcription
72886	2	336302	7	NULL	NULL	0	NULL	Sirt1	GP		inhibits					p53	GP				NULL		0	NULL	NULL	NULL	gw70_annurevpharmacol_45_0_269_s_168	15822178	The human homologue of yeast Sir2a, Sirt1,  inhibits p53 by removing the acetyl group from Lys382 in the C-terminal tail of p53  ( 85).	transcription
72887	3	336302	7	NULL	NULL	0	NULL	statement 2	Process		occur by					p53	GP	removing	acetyl group from Lys382 in the C-terminal tail of		NULL		0	NULL	NULL	NULL	gw70_annurevpharmacol_45_0_269_s_168	15822178	The human homologue of yeast Sir2a, Sirt1,  inhibits p53 by removing the acetyl group from Lys382 in the C-terminal tail of p53  ( 85).	transcription
72903	1	336303	7	NULL	NULL	NULL	NULL	p29ING4	GP		enhance					p53	GP	acetylation of	Lys-382 residue		NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_cancer-res_63_10_12750254_s_6	12750254	p29ING4 and p28ING5 enhance p53 acetylation at Lys-382 residues, and physically  interact with p300, a member of histone acetyl transferase complexes,  and p53 in vivo.	transcription
72904	2	336303	7	NULL	NULL	0	NULL	p28ING5	GP		enhance					p53	GP	acetylation of	Lys-382 residue		NULL		0	NULL	NULL	NULL	abs-batch0650-0679_cancer-res_63_10_12750254_s_6	12750254	p29ING4 and p28ING5 enhance p53 acetylation at Lys-382 residues, and physically  interact with p300, a member of histone acetyl transferase complexes,  and p53 in vivo.	transcription
72905	3	336303	7	NULL	NULL	NULL	NULL	p29ING4	GP		interacts with		physically			p300	GP				NULL	in vivo	NULL	NULL	NULL	NULL	abs-batch0650-0679_cancer-res_63_10_12750254_s_6	12750254	p29ING4 and p28ING5 enhance p53 acetylation at Lys-382 residues, and physically  interact with p300, a member of histone acetyl transferase complexes,  and p53 in vivo.	transcription
72906	4	336303	7	NULL	NULL	NULL	NULL	p28ING5	GP		interacts with		physically			p300	GP				NULL	in vivo	NULL	NULL	NULL	NULL	abs-batch0650-0679_cancer-res_63_10_12750254_s_6	12750254	p29ING4 and p28ING5 enhance p53 acetylation at Lys-382 residues, and physically  interact with p300, a member of histone acetyl transferase complexes,  and p53 in vivo.	transcription
72907	5	336303	7	NULL	NULL	0	NULL	p29ING4	GP		interacts with		physically			p53	GP				NULL	in vivo	0	NULL	NULL	NULL	abs-batch0650-0679_cancer-res_63_10_12750254_s_6	12750254	p29ING4 and p28ING5 enhance p53 acetylation at Lys-382 residues, and physically  interact with p300, a member of histone acetyl transferase complexes,  and p53 in vivo.	transcription
72908	6	336303	7	NULL	NULL	0	NULL	p28ING5	GP		interacts with		physically			p53	GP				NULL	in vivo	0	NULL	NULL	NULL	abs-batch0650-0679_cancer-res_63_10_12750254_s_6	12750254	p29ING4 and p28ING5 enhance p53 acetylation at Lys-382 residues, and physically  interact with p300, a member of histone acetyl transferase complexes,  and p53 in vivo.	transcription
72909	7	336303	7	NULL	NULL	0	NULL	p300	GP		is a type of					histone acetyl transferase complex	GP				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_cancer-res_63_10_12750254_s_6	12750254	p29ING4 and p28ING5 enhance p53 acetylation at Lys-382 residues, and physically  interact with p300, a member of histone acetyl transferase complexes,  and p53 in vivo.	transcription
72910	1	336304	7	NULL	NULL	0	NULL	histone acetyl transferases	GP		recruited to					p53-dependent promoter	GP				NULL		0	NULL	NULL	NULL	gw70_molbiolcell_17_4_1583_s_283	16436515	This modification may contribute to p53 activation by increasing the recruitment of histone acetyl transferases to p53-dependent promoters (Barlev  et al., 2001 ).	transcription
72911	1	336305	7	NULL	NULL	NULL	NULL	p300	GP		bind		stable			p53	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_176	14612423	In the absence of both DNA and acetyl-CoA, the PXXP repeat peptide reduced the stable binding of p300 to p53 (Fig.  3E).	transcription
72912	2	336305	7	NULL	NULL	0	NULL	PXXP repeat peptide	AminoAcid		reduce					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_176	14612423	In the absence of both DNA and acetyl-CoA, the PXXP repeat peptide reduced the stable binding of p300 to p53 (Fig.  3E).	transcription
72913	3	336305	7	NULL	NULL	0	NULL	statement 2	Process		in the absence of					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_176	14612423	In the absence of both DNA and acetyl-CoA, the PXXP repeat peptide reduced the stable binding of p300 to p53 (Fig.  3E).	transcription
72914	4	336305	7	NULL	NULL	0	NULL	statement 2	Process		in the absence of					acetyl-CoA	Chemical				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_176	14612423	In the absence of both DNA and acetyl-CoA, the PXXP repeat peptide reduced the stable binding of p300 to p53 (Fig.  3E).	transcription
72915	1	336306	7	NULL	NULL	0	NULL	p300	GP	full-length	bind					p53	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_47_49395_s_132	15337767	In fact, sequence-specific DNA can stabilize full-length p300 binding to p53 in the absence of acetyl-CoA ( ).	transcription
72916	2	336306	7	NULL	NULL	0	NULL	 DNA	NucleicAcid	sequence-specific	stabilize					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_47_49395_s_132	15337767	In fact, sequence-specific DNA can stabilize full-length p300 binding to p53 in the absence of acetyl-CoA ( ).	transcription
72917	3	336306	7	NULL	NULL	0	NULL	statement 1	Process		in the absence of					acetyl-CoA	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_47_49395_s_132	15337767	In fact, sequence-specific DNA can stabilize full-length p300 binding to p53 in the absence of acetyl-CoA ( ).	transcription
72918	1	336307	7	NULL	NULL	0	NULL	 IFN-alpha	GP		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_17_13547_s_7	11278370	The ability of IFN-alpha and vanadate to induce apoptosis did not require expression of p53 and was blocked by  N-acetyl-L-cysteine.	transcription
72919	2	336307	7	NULL	NULL	0	NULL	vanadate	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_17_13547_s_7	11278370	The ability of IFN-alpha and vanadate to induce apoptosis did not require expression of p53 and was blocked by  N-acetyl-L-cysteine.	transcription
72920	3	336307	7	NULL	NULL	0	NULL	statement 1	Process		does not require					p53	GP	expression of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_17_13547_s_7	11278370	The ability of IFN-alpha and vanadate to induce apoptosis did not require expression of p53 and was blocked by  N-acetyl-L-cysteine.	transcription
72921	4	336307	7	NULL	NULL	0	NULL	N-acetyl-L-cysteine	Chemical		blocks					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_17_13547_s_7	11278370	The ability of IFN-alpha and vanadate to induce apoptosis did not require expression of p53 and was blocked by  N-acetyl-L-cysteine.	transcription
72922	5	336307	7	NULL	NULL	0	NULL	N-acetyl-L-cysteine	Chemical		blocks					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_17_13547_s_7	11278370	The ability of IFN-alpha and vanadate to induce apoptosis did not require expression of p53 and was blocked by  N-acetyl-L-cysteine.	transcription
72923	1	336308	7	NULL	NULL	0	NULL	p300/CBP	GP		recruited to					target gene promoter	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_19_7386_s_23	15123817	First, p300/CBP are recruited by p53 to target gene promoters where they acetylate histones ( ,  ).	transcription
72924	2	336308	7	NULL	NULL	0	NULL	statement 1	Process		recruited by					p53	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_19_7386_s_23	15123817	First, p300/CBP are recruited by p53 to target gene promoters where they acetylate histones ( ,  ).	transcription
72925	1	336309	7	NULL	NULL	0	NULL	PCAF	GP		acetylate					p53	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_200_s_113	11036071	Likewise, PCAF has been shown to acetylate p53, which then increases the DNA binding affinity of p53 ( 36,  37).	transcription
72926	2	336309	7	NULL	NULL	0	NULL	statement 1	Process		increase					p53	GP	DNA binding affinity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_200_s_113	11036071	Likewise, PCAF has been shown to acetylate p53, which then increases the DNA binding affinity of p53 ( 36,  37).	transcription
72927	1	336310	7	NULL	NULL	0	NULL	p53	GP		interacts with					CBP/p300	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1602_1_47_s_166	11960694	The interactions between p53 and CBP/p300 have been associated with subsequent acetylation at the C-terminus of p53 [ 117 and  125], leading to a fairly straightforward model in which stress-induced phosphorylation at the N-terminus of p53 augments interaction with the acetyl-transferases that modify the C-terminus of p53 and activate DNA binding (  Fig. 2).	transcription
72928	2	336310	7	NULL	NULL	NULL	NULL	statement 1	Process		associated with					p53	GP	acetylation at 	C-terminus 		NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1602_1_47_s_166	11960694	The interactions between p53 and CBP/p300 have been associated with subsequent acetylation at the C-terminus of p53 [ 117 and  125], leading to a fairly straightforward model in which stress-induced phosphorylation at the N-terminus of p53 augments interaction with the acetyl-transferases that modify the C-terminus of p53 and activate DNA binding (  Fig. 2).	transcription
72929	3	336310	7	NULL	NULL	0	NULL	stress	Process		induce					p53	GP	phosphorylation of	N-terminus		NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1602_1_47_s_166	11960694	The interactions between p53 and CBP/p300 have been associated with subsequent acetylation at the C-terminus of p53 [ 117 and  125], leading to a fairly straightforward model in which stress-induced phosphorylation at the N-terminus of p53 augments interaction with the acetyl-transferases that modify the C-terminus of p53 and activate DNA binding (  Fig. 2).	transcription
72930	4	336310	7	NULL	NULL	0	NULL	statement 3	Process		augments					acetyl-transferases	GP	interaction with			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1602_1_47_s_166	11960694	The interactions between p53 and CBP/p300 have been associated with subsequent acetylation at the C-terminus of p53 [ 117 and  125], leading to a fairly straightforward model in which stress-induced phosphorylation at the N-terminus of p53 augments interaction with the acetyl-transferases that modify the C-terminus of p53 and activate DNA binding (  Fig. 2).	transcription
72931	5	336310	7	NULL	NULL	0	NULL	statement 4	Process		modify					p53	GP		C-terminus		NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1602_1_47_s_166	11960694	The interactions between p53 and CBP/p300 have been associated with subsequent acetylation at the C-terminus of p53 [ 117 and  125], leading to a fairly straightforward model in which stress-induced phosphorylation at the N-terminus of p53 augments interaction with the acetyl-transferases that modify the C-terminus of p53 and activate DNA binding (  Fig. 2).	transcription
72932	6	336310	7	NULL	NULL	0	NULL	statement 5	Process		activate					DNA binding	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1602_1_47_s_166	11960694	The interactions between p53 and CBP/p300 have been associated with subsequent acetylation at the C-terminus of p53 [ 117 and  125], leading to a fairly straightforward model in which stress-induced phosphorylation at the N-terminus of p53 augments interaction with the acetyl-transferases that modify the C-terminus of p53 and activate DNA binding (  Fig. 2).	transcription
72933	1	336311	7	NULL	NULL	0	NULL	HDAC5	GP		 target of		down-stream			p53	GP				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_cancer-res_62_10_12019172_s_4	12019172	We tested a hypothesis that HDAC5 is a p53  down-stream target gene that on induction by p53 inactivates p53 by removal  of acetyl group in p53 molecule, thus functioning as an auto-regulatory  negative feedback loop in analogue to p53-murine double minute 2 interaction.	transcription
72934	2	336311	7	NULL	NULL	0	NULL	p53	GP		induce					HDAC5	GP				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_cancer-res_62_10_12019172_s_4	12019172	We tested a hypothesis that HDAC5 is a p53  down-stream target gene that on induction by p53 inactivates p53 by removal  of acetyl group in p53 molecule, thus functioning as an auto-regulatory  negative feedback loop in analogue to p53-murine double minute 2 interaction.	transcription
72935	3	336311	7	NULL	NULL	0	NULL	HDAC5	GP		inactivates					p53	GP				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_cancer-res_62_10_12019172_s_4	12019172	We tested a hypothesis that HDAC5 is a p53  down-stream target gene that on induction by p53 inactivates p53 by removal  of acetyl group in p53 molecule, thus functioning as an auto-regulatory  negative feedback loop in analogue to p53-murine double minute 2 interaction.	transcription
72936	4	336311	7	NULL	NULL	0	NULL	statement 3	Process		occur by					p53	GP	removal of	acetyl group		NULL		0	NULL	NULL	NULL	abs-batch0650-0679_cancer-res_62_10_12019172_s_4	12019172	We tested a hypothesis that HDAC5 is a p53  down-stream target gene that on induction by p53 inactivates p53 by removal  of acetyl group in p53 molecule, thus functioning as an auto-regulatory  negative feedback loop in analogue to p53-murine double minute 2 interaction.	transcription
72937	5	336311	7	NULL	NULL	0	NULL	HDAC5	GP		function as					auto-regulatory negative feedback loop	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_cancer-res_62_10_12019172_s_4	12019172	We tested a hypothesis that HDAC5 is a p53  down-stream target gene that on induction by p53 inactivates p53 by removal  of acetyl group in p53 molecule, thus functioning as an auto-regulatory  negative feedback loop in analogue to p53-murine double minute 2 interaction.	transcription
72938	6	336311	7	NULL	NULL	0	NULL	p53	GP		interacts with					murine double minute 2	GP				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_cancer-res_62_10_12019172_s_4	12019172	We tested a hypothesis that HDAC5 is a p53  down-stream target gene that on induction by p53 inactivates p53 by removal  of acetyl group in p53 molecule, thus functioning as an auto-regulatory  negative feedback loop in analogue to p53-murine double minute 2 interaction.	transcription
72939	7	336311	7	NULL	NULL	0	NULL	statement 5	Process		is analogue to					statement 6	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_cancer-res_62_10_12019172_s_4	12019172	We tested a hypothesis that HDAC5 is a p53  down-stream target gene that on induction by p53 inactivates p53 by removal  of acetyl group in p53 molecule, thus functioning as an auto-regulatory  negative feedback loop in analogue to p53-murine double minute 2 interaction.	transcription
72940	1	336312	7	NULL	NULL	0	NULL	 p300	GP		regulator of		important			p53	GP	transcriptional activity of			NULL		0	NULL	NULL	NULL	gw70_pnas_101_33_12165_s_220	15295102	The acetyl-transferase p300 is an important regulator of the transcriptional activity of p53, and disruption of the p300 gene in HCT116 cells demonstrated that p300 also plays important roles for the function of p53  in vivo ( ).	transcription
72941	2	336312	7	NULL	NULL	0	NULL	p300	GP		important role in					p53	GP	function of			NULL	HCT116 cells;;in vivo	0	NULL	NULL	NULL	gw70_pnas_101_33_12165_s_220	15295102	The acetyl-transferase p300 is an important regulator of the transcriptional activity of p53, and disruption of the p300 gene in HCT116 cells demonstrated that p300 also plays important roles for the function of p53  in vivo ( ).	transcription
72942	3	336312	7	NULL	NULL	0	NULL	p300	GP		is a type of					acetyl-transferase	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_33_12165_s_220	15295102	The acetyl-transferase p300 is an important regulator of the transcriptional activity of p53, and disruption of the p300 gene in HCT116 cells demonstrated that p300 also plays important roles for the function of p53  in vivo ( ).	transcription
72943	1	336313	7	NULL	NULL	NULL	NULL	LMB	Chemical		induce					p53	GP	accumulation of			NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_24_7_1177_s_6	12807744	Caffeine inhibited the accumulation of p53 induced by leptomycin B (LMB), an inhibitor of CRM1, but not  N-acetyl-leu-leu-norleucinal, a proteasome inhibitor.	transcription
72944	2	336313	7	NULL	NULL	0	NULL	Caffeine	Chemical		inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_24_7_1177_s_6	12807744	Caffeine inhibited the accumulation of p53 induced by leptomycin B (LMB), an inhibitor of CRM1, but not  N-acetyl-leu-leu-norleucinal, a proteasome inhibitor.	transcription
72945	3	336313	7	NULL	NULL	0	NULL	LMB	Chemical		inhibitor of					CRM1	Chemical				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_24_7_1177_s_6	12807744	Caffeine inhibited the accumulation of p53 induced by leptomycin B (LMB), an inhibitor of CRM1, but not  N-acetyl-leu-leu-norleucinal, a proteasome inhibitor.	transcription
72946	4	336313	7	NULL	NULL	0	NULL	N-acetyl-leu-leu-norleucinal	Chemical		induce					p53	GP	accumulation of			NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_24_7_1177_s_6	12807744	Caffeine inhibited the accumulation of p53 induced by leptomycin B (LMB), an inhibitor of CRM1, but not  N-acetyl-leu-leu-norleucinal, a proteasome inhibitor.	transcription
72947	5	336313	7	NULL	NULL	NULL	NULL	Caffeine	Chemical		does not inhibit					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_24_7_1177_s_6	12807744	Caffeine inhibited the accumulation of p53 induced by leptomycin B (LMB), an inhibitor of CRM1, but not  N-acetyl-leu-leu-norleucinal, a proteasome inhibitor.	transcription
72948	6	336313	7	NULL	NULL	0	NULL	N-acetyl-leu-leu-norleucinal	Chemical		is a inhibitor of					proteasome	CellComponent				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_24_7_1177_s_6	12807744	Caffeine inhibited the accumulation of p53 induced by leptomycin B (LMB), an inhibitor of CRM1, but not  N-acetyl-leu-leu-norleucinal, a proteasome inhibitor.	transcription
72949	7	336313	7	NULL	NULL	0	NULL	LMB	Chemical		is					 leptomycin B	Chemical				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_24_7_1177_s_6	12807744	Caffeine inhibited the accumulation of p53 induced by leptomycin B (LMB), an inhibitor of CRM1, but not  N-acetyl-leu-leu-norleucinal, a proteasome inhibitor.	transcription
72950	1	336314	7	NULL	NULL	0	NULL	N-acetyl-L-cysteine	Chemical	dietary	modulates					benzo[apyrene-induced skin tumors	MedicalFinding				NULL	cancer-prone p53 haploinsufficient Tg.AC (v-Ha-ras) mice	0	NULL	NULL	NULL	gw70_annurevnutr_24_0_223_s_697	15189120	Dietary  N-acetyl-L-cysteine modulates benzo[apyrene-induced skin tumors in cancer-prone  p53 haploinsufficient Tg.AC (v-Ha-ras) mice.	transcription
72951	1	336315	7	NULL	NULL	NULL	NULL	CobB protein	GP	Salmonella	deacetylates					acetyl-coenzyme A synthetase	GP		active site of		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_3_1301_s_18	14729974	The CobB protein of  Salmonella deacetylates the active site of acetyl-coenzyme A synthetase ( ), mammalian SIRT1 deacetylates the p53 tumor suppressor protein ( ,  ,  ), and human SIRT2 deacetylates tubulin ( ).	transcription
72952	2	336315	7	NULL	NULL	0	NULL	SIRT1	GP	mammalian	deacetylates					p53	GP				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1301_s_18	14729974	The CobB protein of  Salmonella deacetylates the active site of acetyl-coenzyme A synthetase ( ), mammalian SIRT1 deacetylates the p53 tumor suppressor protein ( ,  ,  ), and human SIRT2 deacetylates tubulin ( ).	transcription
72953	3	336315	7	NULL	NULL	0	NULL	 SIRT2 	GP	human	deacetylates					tubulin	GP				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1301_s_18	14729974	The CobB protein of  Salmonella deacetylates the active site of acetyl-coenzyme A synthetase ( ), mammalian SIRT1 deacetylates the p53 tumor suppressor protein ( ,  ,  ), and human SIRT2 deacetylates tubulin ( ).	transcription
72954	4	336315	7	NULL	NULL	0	NULL	p53	GP		is a type of					tumor suppressor protein	GP				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_3_1301_s_18	14729974	The CobB protein of  Salmonella deacetylates the active site of acetyl-coenzyme A synthetase ( ), mammalian SIRT1 deacetylates the p53 tumor suppressor protein ( ,  ,  ), and human SIRT2 deacetylates tubulin ( ).	transcription
72955	1	336316	7	NULL	NULL	0	NULL	BPDE	Chemical		induce					p53	GP	accumulation of			NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_27_3_631_s_152	16244358	Next, we examined whether p53 accumulation and phosphorylation are also induced by proteasomal inhibitor  N-Acetyl-Leu-Leu-Nle-CHO (ALLN) (Calbiochem) in order to compare with BPDE-induced p53 accumulation and phosphorylation, and whether TPA can attenuate ALLN-induced p53 accumulation and phosphorylation, if they occurred.	transcription
72956	2	336316	7	NULL	NULL	0	NULL	BPDE	Chemical		induce					p53	GP	phosphorylation of			NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_27_3_631_s_152	16244358	Next, we examined whether p53 accumulation and phosphorylation are also induced by proteasomal inhibitor  N-Acetyl-Leu-Leu-Nle-CHO (ALLN) (Calbiochem) in order to compare with BPDE-induced p53 accumulation and phosphorylation, and whether TPA can attenuate ALLN-induced p53 accumulation and phosphorylation, if they occurred.	transcription
72957	3	336316	7	NULL	NULL	0	NULL	ALLN	Chemical		induce					p53	GP	accumulation of			NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_27_3_631_s_152	16244358	Next, we examined whether p53 accumulation and phosphorylation are also induced by proteasomal inhibitor  N-Acetyl-Leu-Leu-Nle-CHO (ALLN) (Calbiochem) in order to compare with BPDE-induced p53 accumulation and phosphorylation, and whether TPA can attenuate ALLN-induced p53 accumulation and phosphorylation, if they occurred.	transcription
72958	4	336316	7	NULL	NULL	0	NULL	ALLN	Chemical		induce					p53	GP	phosphorylation of			NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_27_3_631_s_152	16244358	Next, we examined whether p53 accumulation and phosphorylation are also induced by proteasomal inhibitor  N-Acetyl-Leu-Leu-Nle-CHO (ALLN) (Calbiochem) in order to compare with BPDE-induced p53 accumulation and phosphorylation, and whether TPA can attenuate ALLN-induced p53 accumulation and phosphorylation, if they occurred.	transcription
72959	5	336316	7	NULL	NULL	0	NULL	ALLN	Chemical		is					N-Acetyl-Leu-Leu-Nle-CHO	Chemical				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_27_3_631_s_152	16244358	Next, we examined whether p53 accumulation and phosphorylation are also induced by proteasomal inhibitor  N-Acetyl-Leu-Leu-Nle-CHO (ALLN) (Calbiochem) in order to compare with BPDE-induced p53 accumulation and phosphorylation, and whether TPA can attenuate ALLN-induced p53 accumulation and phosphorylation, if they occurred.	transcription
72960	6	336316	7	NULL	NULL	0	NULL	ALLN	Chemical		is a type of					proteasomal inhibitor	Chemical				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_27_3_631_s_152	16244358	Next, we examined whether p53 accumulation and phosphorylation are also induced by proteasomal inhibitor  N-Acetyl-Leu-Leu-Nle-CHO (ALLN) (Calbiochem) in order to compare with BPDE-induced p53 accumulation and phosphorylation, and whether TPA can attenuate ALLN-induced p53 accumulation and phosphorylation, if they occurred.	transcription
72961	1	336317	7	NULL	NULL	NULL	NULL	p53	GP	phosphorylation within	stimulate			N-terminus		p53	GP	transcriptional activity of			NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1602_1_47_s_165	11960694	Phosphorylation within the N-terminus of p53 can stimulate p53's transcriptional activity without influencing MDM2 binding, and both serine 15 and serine 33 phosphorylation leads to enhanced binding between p53 and histone acetyl transferases such as p300/CBP or pCAF [  123,   124 and   125].	transcription
72962	2	336317	7	NULL	NULL	0	NULL	statement 1	Process		does not influence					MDM2	GP	binding of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1602_1_47_s_165	11960694	Phosphorylation within the N-terminus of p53 can stimulate p53's transcriptional activity without influencing MDM2 binding, and both serine 15 and serine 33 phosphorylation leads to enhanced binding between p53 and histone acetyl transferases such as p300/CBP or pCAF [  123,   124 and   125].	transcription
72963	3	336317	7	NULL	NULL	0	NULL	p53	GP		bind					p300/CBP	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1602_1_47_s_165	11960694	Phosphorylation within the N-terminus of p53 can stimulate p53's transcriptional activity without influencing MDM2 binding, and both serine 15 and serine 33 phosphorylation leads to enhanced binding between p53 and histone acetyl transferases such as p300/CBP or pCAF [  123,   124 and   125].	transcription
72964	4	336317	7	NULL	NULL	0	NULL	p53	GP		bind					pCAF	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1602_1_47_s_165	11960694	Phosphorylation within the N-terminus of p53 can stimulate p53's transcriptional activity without influencing MDM2 binding, and both serine 15 and serine 33 phosphorylation leads to enhanced binding between p53 and histone acetyl transferases such as p300/CBP or pCAF [  123,   124 and   125].	transcription
72965	5	336317	7	NULL	NULL	0	NULL	p53	GP	phosphorylation of	enhance			serine 15		statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1602_1_47_s_165	11960694	Phosphorylation within the N-terminus of p53 can stimulate p53's transcriptional activity without influencing MDM2 binding, and both serine 15 and serine 33 phosphorylation leads to enhanced binding between p53 and histone acetyl transferases such as p300/CBP or pCAF [  123,   124 and   125].	transcription
72966	6	336317	7	NULL	NULL	NULL	NULL	p53	GP	phosphorylation of	enhance			serine 33		statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1602_1_47_s_165	11960694	Phosphorylation within the N-terminus of p53 can stimulate p53's transcriptional activity without influencing MDM2 binding, and both serine 15 and serine 33 phosphorylation leads to enhanced binding between p53 and histone acetyl transferases such as p300/CBP or pCAF [  123,   124 and   125].	transcription
72967	7	336317	7	NULL	NULL	0	NULL	p53	GP	phosphorylation of	enhance			serine 15		statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1602_1_47_s_165	11960694	Phosphorylation within the N-terminus of p53 can stimulate p53's transcriptional activity without influencing MDM2 binding, and both serine 15 and serine 33 phosphorylation leads to enhanced binding between p53 and histone acetyl transferases such as p300/CBP or pCAF [  123,   124 and   125].	transcription
72968	8	336317	7	NULL	NULL	0	NULL	p53	GP	phosphorylation of	enhance			serine 33		statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1602_1_47_s_165	11960694	Phosphorylation within the N-terminus of p53 can stimulate p53's transcriptional activity without influencing MDM2 binding, and both serine 15 and serine 33 phosphorylation leads to enhanced binding between p53 and histone acetyl transferases such as p300/CBP or pCAF [  123,   124 and   125].	transcription
72969	9	336317	7	NULL	NULL	0	NULL	p300/CBP	GP		is a type of					histone acetyl transferases	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1602_1_47_s_165	11960694	Phosphorylation within the N-terminus of p53 can stimulate p53's transcriptional activity without influencing MDM2 binding, and both serine 15 and serine 33 phosphorylation leads to enhanced binding between p53 and histone acetyl transferases such as p300/CBP or pCAF [  123,   124 and   125].	transcription
72970	10	336317	7	NULL	NULL	0	NULL	pCAF	GP		is a type of					histone acetyl transferases	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1602_1_47_s_165	11960694	Phosphorylation within the N-terminus of p53 can stimulate p53's transcriptional activity without influencing MDM2 binding, and both serine 15 and serine 33 phosphorylation leads to enhanced binding between p53 and histone acetyl transferases such as p300/CBP or pCAF [  123,   124 and   125].	transcription
72971	1	336318	7	NULL	NULL	0	NULL	p300	GP		acetylates					p53	GP		C terminus		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_48_47853_s_265	14500729	p300 acetylates the C terminus of p53, leading to transcriptional activation of p53 function ( ,  ).	transcription
72972	2	336318	7	NULL	NULL	0	NULL	statement 1	Process		leads to					p53 function	Process	transcriptional activation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_48_47853_s_265	14500729	p300 acetylates the C terminus of p53, leading to transcriptional activation of p53 function ( ,  ).	transcription
72973	1	336319	7	NULL	NULL	0	NULL	IE2	GP		downregulate		could			p53 function	Process				NULL		0	NULL	NULL	NULL	gw70_embo_23_11_2269_s_211	15141169	Thus far, we had demonstrated that IE2 could downregulate p53 function and inhibit  the acetylase activity of the p53 coactivators, p300/CBP, both  in vitro and  in vivo.	transcription
72974	2	336319	7	NULL	NULL	NULL	NULL	statement 1	Process		inhibit					p53 coactivators	GP	acetylase activity of			NULL	in vitro	NULL	NULL	NULL	NULL	gw70_embo_23_11_2269_s_211	15141169	Thus far, we had demonstrated that IE2 could downregulate p53 function and inhibit  the acetylase activity of the p53 coactivators, p300/CBP, both  in vitro and  in vivo.	transcription
72975	3	336319	7	NULL	NULL	NULL	NULL	statement 1	Process		inhibit					p53 coactivators	GP	acetylase activity of			NULL	in vivo	NULL	NULL	NULL	NULL	gw70_embo_23_11_2269_s_211	15141169	Thus far, we had demonstrated that IE2 could downregulate p53 function and inhibit  the acetylase activity of the p53 coactivators, p300/CBP, both  in vitro and  in vivo.	transcription
72976	4	336319	7	NULL	NULL	0	NULL	statement 1	Process		inhibit					 p300/CBP	GP				NULL	in vitro	0	NULL	NULL	NULL	gw70_embo_23_11_2269_s_211	15141169	Thus far, we had demonstrated that IE2 could downregulate p53 function and inhibit  the acetylase activity of the p53 coactivators, p300/CBP, both  in vitro and  in vivo.	transcription
72977	5	336319	7	NULL	NULL	0	NULL	statement 1	Process		inhibit					p300/CBP	GP				NULL	in vivo	0	NULL	NULL	NULL	gw70_embo_23_11_2269_s_211	15141169	Thus far, we had demonstrated that IE2 could downregulate p53 function and inhibit  the acetylase activity of the p53 coactivators, p300/CBP, both  in vitro and  in vivo.	transcription
72978	1	336320	7	NULL	NULL	0	NULL				interacts with			Tat domain					HAT domain		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_9390_s_100	15611041	Since we have previously demonstrated that Tat-HAT domain interactions prevent coactivator-mediated acetylation of the tumor suppressor p53 ( ), we investigated whether Tat-coactivator binding might inhibit histone acetylation by p300 and PCAF in radioactive acetylation assays using [14]acetyl-coenzyme A (acetyl-CoA).	transcription
72979	2	336320	7	NULL	NULL	0	NULL	coactivator	GP		mediate					p53	GP	acetylation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_9390_s_100	15611041	Since we have previously demonstrated that Tat-HAT domain interactions prevent coactivator-mediated acetylation of the tumor suppressor p53 ( ), we investigated whether Tat-coactivator binding might inhibit histone acetylation by p300 and PCAF in radioactive acetylation assays using [14]acetyl-coenzyme A (acetyl-CoA).	transcription
72980	3	336320	7	NULL	NULL	0	NULL	p53	GP		is a type of					tumor suppressor	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_9390_s_100	15611041	Since we have previously demonstrated that Tat-HAT domain interactions prevent coactivator-mediated acetylation of the tumor suppressor p53 ( ), we investigated whether Tat-coactivator binding might inhibit histone acetylation by p300 and PCAF in radioactive acetylation assays using [14]acetyl-coenzyme A (acetyl-CoA).	transcription
72981	4	336320	7	NULL	NULL	0	NULL	statement 1	Process		prevent					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_10_9390_s_100	15611041	Since we have previously demonstrated that Tat-HAT domain interactions prevent coactivator-mediated acetylation of the tumor suppressor p53 ( ), we investigated whether Tat-coactivator binding might inhibit histone acetylation by p300 and PCAF in radioactive acetylation assays using [14]acetyl-coenzyme A (acetyl-CoA).	transcription
72982	1	336321	7	NULL	NULL	0	NULL	p300	GP		bind					p53	GP				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_18_2831_s_94	9744860	Although a small amount of binding was observed either when acetyl-CoA was omitted or when it was replaced by unacetylated CoA (Fig.  5, lanes 7,8,11,12), this amount was substantially less than in the presence of acetyl-CoA, indicating that acetylation and not simply binding of either p300 or PCAF to p53 was necessary for the effect on DNA-binding.	transcription
72983	2	336321	7	NULL	NULL	0	NULL	PCAF	GP		bind					p53	GP				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_18_2831_s_94	9744860	Although a small amount of binding was observed either when acetyl-CoA was omitted or when it was replaced by unacetylated CoA (Fig.  5, lanes 7,8,11,12), this amount was substantially less than in the presence of acetyl-CoA, indicating that acetylation and not simply binding of either p300 or PCAF to p53 was necessary for the effect on DNA-binding.	transcription
72984	3	336321	7	NULL	NULL	0	NULL	p53	GP		bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_18_2831_s_94	9744860	Although a small amount of binding was observed either when acetyl-CoA was omitted or when it was replaced by unacetylated CoA (Fig.  5, lanes 7,8,11,12), this amount was substantially less than in the presence of acetyl-CoA, indicating that acetylation and not simply binding of either p300 or PCAF to p53 was necessary for the effect on DNA-binding.	transcription
72985	4	336321	7	NULL	NULL	0	NULL	acetyl-CoA	Chemical	acetylation by	is necessary for					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_18_2831_s_94	9744860	Although a small amount of binding was observed either when acetyl-CoA was omitted or when it was replaced by unacetylated CoA (Fig.  5, lanes 7,8,11,12), this amount was substantially less than in the presence of acetyl-CoA, indicating that acetylation and not simply binding of either p300 or PCAF to p53 was necessary for the effect on DNA-binding.	transcription
72986	5	336321	7	NULL	NULL	NULL	NULL	statement 1	Process		not required for					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_12_18_2831_s_94	9744860	Although a small amount of binding was observed either when acetyl-CoA was omitted or when it was replaced by unacetylated CoA (Fig.  5, lanes 7,8,11,12), this amount was substantially less than in the presence of acetyl-CoA, indicating that acetylation and not simply binding of either p300 or PCAF to p53 was necessary for the effect on DNA-binding.	transcription
72987	6	336321	7	NULL	NULL	0	NULL	statement 2	Process		not required for					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_genesdev_12_18_2831_s_94	9744860	Although a small amount of binding was observed either when acetyl-CoA was omitted or when it was replaced by unacetylated CoA (Fig.  5, lanes 7,8,11,12), this amount was substantially less than in the presence of acetyl-CoA, indicating that acetylation and not simply binding of either p300 or PCAF to p53 was necessary for the effect on DNA-binding.	transcription
72988	1	336322	7	NULL	NULL	0	NULL	CBP/p300	GP		acetylate					p53	GP				NULL		0	NULL	NULL	NULL	gw70_annurevgenet_34_0_77_s_284	11092823	Acetylation by CBP/p300 and PCAF both enhance p53's DNA-binding activity even  though the two factors acetylate different sites on p53.	transcription
72989	2	336322	7	NULL	NULL	0	NULL	PCAF	GP		acetylate					p53	GP				NULL		0	NULL	NULL	NULL	gw70_annurevgenet_34_0_77_s_284	11092823	Acetylation by CBP/p300 and PCAF both enhance p53's DNA-binding activity even  though the two factors acetylate different sites on p53.	transcription
72990	3	336322	7	NULL	NULL	0	NULL	p53	GP		bind					DNA 	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_annurevgenet_34_0_77_s_284	11092823	Acetylation by CBP/p300 and PCAF both enhance p53's DNA-binding activity even  though the two factors acetylate different sites on p53.	transcription
72991	4	336322	7	NULL	NULL	0	NULL	statement 1	Process		enhance					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_annurevgenet_34_0_77_s_284	11092823	Acetylation by CBP/p300 and PCAF both enhance p53's DNA-binding activity even  though the two factors acetylate different sites on p53.	transcription
72992	5	336322	7	NULL	NULL	0	NULL	statement 2	Process		enhance					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_annurevgenet_34_0_77_s_284	11092823	Acetylation by CBP/p300 and PCAF both enhance p53's DNA-binding activity even  though the two factors acetylate different sites on p53.	transcription
72993	6	336322	7	NULL	NULL	0	NULL	statement 1	GP	acetylation site of	is different from					statement 2	GP	acetylation site of			NULL		0	NULL	NULL	NULL	gw70_annurevgenet_34_0_77_s_284	11092823	Acetylation by CBP/p300 and PCAF both enhance p53's DNA-binding activity even  though the two factors acetylate different sites on p53.	transcription
72994	1	336323	7	NULL	NULL	0	NULL	p300/CBP	GP		acetylate					p53	GP		lysine residues within C terminus		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20111_s_40	15769743	In addition, p300/CBP is found to acetylate several lysine residues within the p53 C terminus, which enhances the DNA binding and thereby the transcriptional activity of p53 ( ,  ,   -  ).	transcription
72995	2	336323	7	NULL	NULL	0	NULL	p53	GP		bind					DNA	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20111_s_40	15769743	In addition, p300/CBP is found to acetylate several lysine residues within the p53 C terminus, which enhances the DNA binding and thereby the transcriptional activity of p53 ( ,  ,   -  ).	transcription
72996	3	336323	7	NULL	NULL	0	NULL	statement 1	Process		enhance					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20111_s_40	15769743	In addition, p300/CBP is found to acetylate several lysine residues within the p53 C terminus, which enhances the DNA binding and thereby the transcriptional activity of p53 ( ,  ,   -  ).	transcription
72997	4	336323	7	NULL	NULL	0	NULL	statement 3	Process		enhance					p53	GP	transcriptional activity of 			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_20_20111_s_40	15769743	In addition, p300/CBP is found to acetylate several lysine residues within the p53 C terminus, which enhances the DNA binding and thereby the transcriptional activity of p53 ( ,  ,   -  ).	transcription
72998	1	336324	7	NULL	NULL	0	NULL	p53	GP		interacts with					p300	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_39115_s_5	11495913	Furthermore, interaction of p53 with the transcriptional coactivator p300 was induced, and Lys382 of p53 was acetylated.	transcription
72999	2	336324	7	NULL	NULL	0	NULL	p300	GP		is a type of					transcriptional coactivator	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_42_39115_s_5	11495913	Furthermore, interaction of p53 with the transcriptional coactivator p300 was induced, and Lys382 of p53 was acetylated.	transcription
73000	1	336325	7	NULL	NULL	0	NULL	RA	Chemical		induce					p53	GP				NULL		0	NULL	NULL	NULL	gw70_embo_25_17_4084_s_120	16946709	Despite the lower p53 levels induced by RA, acetylation of K320 but not of K372  of p53 was markedly increased, and RA treatment also clearly induced the expression  levels of the acetyltransferase PCAF, which is known to acetylate p53 at K320 (  et al).	transcription
73001	2	336325	7	NULL	NULL	0	NULL	statement 1	Process		increase					p53	GP	acetylation of	K320		NULL		0	NULL	NULL	NULL	gw70_embo_25_17_4084_s_120	16946709	Despite the lower p53 levels induced by RA, acetylation of K320 but not of K372  of p53 was markedly increased, and RA treatment also clearly induced the expression  levels of the acetyltransferase PCAF, which is known to acetylate p53 at K320 (  et al).	transcription
73002	3	336325	7	NULL	NULL	0	NULL	statement 1	Process		does not increase					p53	GP		K372		NULL		0	NULL	NULL	NULL	gw70_embo_25_17_4084_s_120	16946709	Despite the lower p53 levels induced by RA, acetylation of K320 but not of K372  of p53 was markedly increased, and RA treatment also clearly induced the expression  levels of the acetyltransferase PCAF, which is known to acetylate p53 at K320 (  et al).	transcription
73003	4	336325	7	NULL	NULL	0	NULL	RA	Chemical		induce					 PCAF	GP	expression of			NULL		0	NULL	NULL	NULL	gw70_embo_25_17_4084_s_120	16946709	Despite the lower p53 levels induced by RA, acetylation of K320 but not of K372  of p53 was markedly increased, and RA treatment also clearly induced the expression  levels of the acetyltransferase PCAF, which is known to acetylate p53 at K320 (  et al).	transcription
73004	5	336325	7	NULL	NULL	0	NULL	PCAF	GP		acetylate					p53	GP		K320		NULL		0	NULL	NULL	NULL	gw70_embo_25_17_4084_s_120	16946709	Despite the lower p53 levels induced by RA, acetylation of K320 but not of K372  of p53 was markedly increased, and RA treatment also clearly induced the expression  levels of the acetyltransferase PCAF, which is known to acetylate p53 at K320 (  et al).	transcription
73005	6	336325	7	NULL	NULL	0	NULL	PCAF	GP		is a type of					acetyltransferase	GP				NULL		0	NULL	NULL	NULL	gw70_embo_25_17_4084_s_120	16946709	Despite the lower p53 levels induced by RA, acetylation of K320 but not of K372  of p53 was markedly increased, and RA treatment also clearly induced the expression  levels of the acetyltransferase PCAF, which is known to acetylate p53 at K320 (  et al).	transcription
73006	1	336326	7	NULL	NULL	0	NULL	p300	GP		bind					anti-p300 serum	GP				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_22_10083_s_258	15509808	(C) Acetylation reactions were carried out as described above but in the absence  of acetyl-CoA; p300 binding was determined by ELISA with anti-p300 serum (N15) following  capture of p53 by using ICA-9.	transcription
73007	1	336327	7	NULL	NULL	0	NULL	 reoxygenation	Process		induce					p53	GP	phosphorylation of	serine 15		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_14_12207_s_9	12519769	The reoxygenation-induced p53 serine 15 phosphorylation was inhibited by the addition of  N-acetyl-L-cysteine (NAC), indicating that free radical-induced DNA damage was mediated by reactive oxygen species.	transcription
73008	2	336327	7	NULL	NULL	0	NULL	NAC	Chemical		inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_14_12207_s_9	12519769	The reoxygenation-induced p53 serine 15 phosphorylation was inhibited by the addition of  N-acetyl-L-cysteine (NAC), indicating that free radical-induced DNA damage was mediated by reactive oxygen species.	transcription
73009	3	336327	7	NULL	NULL	0	NULL	free radical	Chemical		induce					DNA damage	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_14_12207_s_9	12519769	The reoxygenation-induced p53 serine 15 phosphorylation was inhibited by the addition of  N-acetyl-L-cysteine (NAC), indicating that free radical-induced DNA damage was mediated by reactive oxygen species.	transcription
73010	4	336327	7	NULL	NULL	0	NULL	reactive oxygen species	Chemical		mediate					statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_14_12207_s_9	12519769	The reoxygenation-induced p53 serine 15 phosphorylation was inhibited by the addition of  N-acetyl-L-cysteine (NAC), indicating that free radical-induced DNA damage was mediated by reactive oxygen species.	transcription
73011	5	336327	7	NULL	NULL	0	NULL	NAC	Chemical		is					N-acetyl-L-cysteine	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_14_12207_s_9	12519769	The reoxygenation-induced p53 serine 15 phosphorylation was inhibited by the addition of  N-acetyl-L-cysteine (NAC), indicating that free radical-induced DNA damage was mediated by reactive oxygen species.	transcription
73012	6	336327	7	NULL	NULL	0	NULL	statement 2	Process		indicate					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_14_12207_s_9	12519769	The reoxygenation-induced p53 serine 15 phosphorylation was inhibited by the addition of  N-acetyl-L-cysteine (NAC), indicating that free radical-induced DNA damage was mediated by reactive oxygen species.	transcription
73013	1	336328	7	NULL	NULL	0	NULL	 N-acetyl-L-cysteine	GP		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_circulation_105_1_79_s_170	11772880	28 Interestingly, the induction of apoptosis by  N-acetyl-L-cysteine has also been linked to an increase in p53 expression, 29 suggesting that antioxidants stimulate apoptosis via a p53-dependent pathway.	transcription
73014	2	336328	7	NULL	NULL	0	NULL	statement 1	Process		linked to					p53	GP	increased expression of			NULL		0	NULL	NULL	NULL	gw60_circulation_105_1_79_s_170	11772880	28 Interestingly, the induction of apoptosis by  N-acetyl-L-cysteine has also been linked to an increase in p53 expression, 29 suggesting that antioxidants stimulate apoptosis via a p53-dependent pathway.	transcription
73015	3	336328	7	NULL	NULL	0	NULL	antioxidants	Process		stimulate					apoptosis	Process				NULL		0	NULL	NULL	NULL	gw60_circulation_105_1_79_s_170	11772880	28 Interestingly, the induction of apoptosis by  N-acetyl-L-cysteine has also been linked to an increase in p53 expression, 29 suggesting that antioxidants stimulate apoptosis via a p53-dependent pathway.	transcription
73016	4	336328	7	NULL	NULL	0	NULL	statement 2	Process		via					p53 dependent pathway	Process				NULL		0	NULL	NULL	NULL	gw60_circulation_105_1_79_s_170	11772880	28 Interestingly, the induction of apoptosis by  N-acetyl-L-cysteine has also been linked to an increase in p53 expression, 29 suggesting that antioxidants stimulate apoptosis via a p53-dependent pathway.	transcription
73017	5	336328	7	NULL	NULL	0	NULL	statement 2	Process		suggest					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_circulation_105_1_79_s_170	11772880	28 Interestingly, the induction of apoptosis by  N-acetyl-L-cysteine has also been linked to an increase in p53 expression, 29 suggesting that antioxidants stimulate apoptosis via a p53-dependent pathway.	transcription
73018	1	336329	7	NULL	NULL	0	NULL	acetyl-CoA	Chemical		stimulate		greatly			p53	GP	binding of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_2_1202_s_155	9891054	The addition of acetyl-CoA and PCAF greatly stimulated the binding of p53, both in the presence and absence of PAb421 (Fig.  5, compare lanes 2 and 3 to lanes 9 and 10).	transcription
73019	2	336329	7	NULL	NULL	0	NULL	PCAF	GP		stimulate		greatly			p53	GP	binding of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_2_1202_s_155	9891054	The addition of acetyl-CoA and PCAF greatly stimulated the binding of p53, both in the presence and absence of PAb421 (Fig.  5, compare lanes 2 and 3 to lanes 9 and 10).	transcription
73020	1	336330	7	NULL	NULL	0	NULL	p300	GP		complex with					p53	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_15_13431_s_261	12499368	The stability of the p300.p53 complex was therefore quantitated without or with acetyl-CoA using the ELISA solid phase assay to determine whether p300 dissociates from p53 after acetylation in the absence or presence of consensus site DNA.	transcription
73021	1	336331	7	NULL	NULL	0	NULL	p300	GP		bind					p53	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_15_13431_s_265	12499368	Furthermore, p300 binding to p53 (Fig.  9,  lane 5) was de-stabilized by acetyl-CoA in reactions with nonspecific DNA (Fig.  9,  A and  B,  lane 11 versus 5).	transcription
73022	2	336331	7	NULL	NULL	NULL	NULL	acetyl-CoA	Chemical		in reactions with					nonspecific DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_15_13431_s_265	12499368	Furthermore, p300 binding to p53 (Fig.  9,  lane 5) was de-stabilized by acetyl-CoA in reactions with nonspecific DNA (Fig.  9,  A and  B,  lane 11 versus 5).	transcription
73023	3	336331	7	NULL	NULL	0	NULL	statement 2	Process		destabilize					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_15_13431_s_265	12499368	Furthermore, p300 binding to p53 (Fig.  9,  lane 5) was de-stabilized by acetyl-CoA in reactions with nonspecific DNA (Fig.  9,  A and  B,  lane 11 versus 5).	transcription
73024	1	336333	7	NULL	NULL	0	NULL	E2F1	GP		interacts with					HBx	GP				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_iubmb-life_53_6_12625370_s_2	12625370	The functional effect of the interaction of E2F1 and hepatitis B virus  X protein (HBx) on the promoter of human p53 gene was studied using chloramphenicol  acetyl transferase (CAT) assay.	transcription
73025	2	336333	7	NULL	NULL	0	NULL	HBx	GP		present on					p53 gene	GP	human		promoter	NULL		0	NULL	NULL	NULL	abs-batch0650-0679_iubmb-life_53_6_12625370_s_2	12625370	The functional effect of the interaction of E2F1 and hepatitis B virus  X protein (HBx) on the promoter of human p53 gene was studied using chloramphenicol  acetyl transferase (CAT) assay.	transcription
73026	3	336333	7	NULL	NULL	0	NULL	HBx	GP		is					hepatitis B virus X protein	GP				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_iubmb-life_53_6_12625370_s_2	12625370	The functional effect of the interaction of E2F1 and hepatitis B virus  X protein (HBx) on the promoter of human p53 gene was studied using chloramphenicol  acetyl transferase (CAT) assay.	transcription
73027	1	336334	7	NULL	NULL	0	NULL	coactivator	GP	recruitment of	depends on					p53	GP	acetylation of			NULL		0	NULL	NULL	NULL	abs-batch0650-0679_mol-cell_13_2_14759370_s_4	14759370	This bromodomain/acetyl-lysine binding  is responsible for p53 acetylation-dependent coactivator recruitment after  DNA damage, a step essential for p53-induced transcriptional activation  of the cyclin-dependent kinase inhibitor p21 in G1 cell cycle arrest.	transcription
73028	2	336334	7	NULL	NULL	0	NULL	statement 1	Process		occur after					DNA damage	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_mol-cell_13_2_14759370_s_4	14759370	This bromodomain/acetyl-lysine binding  is responsible for p53 acetylation-dependent coactivator recruitment after  DNA damage, a step essential for p53-induced transcriptional activation  of the cyclin-dependent kinase inhibitor p21 in G1 cell cycle arrest.	transcription
73029	3	336334	7	NULL	NULL	0	NULL	bromodomain/acetyl-lysine	Chemical	binding of	is responsible for					statement 1	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_mol-cell_13_2_14759370_s_4	14759370	This bromodomain/acetyl-lysine binding  is responsible for p53 acetylation-dependent coactivator recruitment after  DNA damage, a step essential for p53-induced transcriptional activation  of the cyclin-dependent kinase inhibitor p21 in G1 cell cycle arrest.	transcription
73030	4	336334	7	NULL	NULL	NULL	NULL	p53	GP		induce					p21	GP	transcriptional activation of			NULL		NULL	NULL	NULL	NULL	abs-batch0650-0679_mol-cell_13_2_14759370_s_4	14759370	This bromodomain/acetyl-lysine binding  is responsible for p53 acetylation-dependent coactivator recruitment after  DNA damage, a step essential for p53-induced transcriptional activation  of the cyclin-dependent kinase inhibitor p21 in G1 cell cycle arrest.	transcription
73031	5	336334	7	NULL	NULL	0	NULL	statement 4	Process		occur in					G1 cell cycle arrest	Process				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_mol-cell_13_2_14759370_s_4	14759370	This bromodomain/acetyl-lysine binding  is responsible for p53 acetylation-dependent coactivator recruitment after  DNA damage, a step essential for p53-induced transcriptional activation  of the cyclin-dependent kinase inhibitor p21 in G1 cell cycle arrest.	transcription
73032	6	336334	7	NULL	NULL	0	NULL	p21	GP		is a type of					cyclin-dependent kinase inhibitor	GP				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_mol-cell_13_2_14759370_s_4	14759370	This bromodomain/acetyl-lysine binding  is responsible for p53 acetylation-dependent coactivator recruitment after  DNA damage, a step essential for p53-induced transcriptional activation  of the cyclin-dependent kinase inhibitor p21 in G1 cell cycle arrest.	transcription
73033	1	336335	7	NULL	NULL	0	NULL	p53	GP		bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_1_118_s_36	12147236	By using a acetylase defective mutant of CBP (L1690K/C1691L), we have found that the acetylase activity of CBP is not required for stimulation of p53 DNA binding (unpublished data).	transcription
73034	2	336335	7	NULL	NULL	0	NULL	CBP 	GP	acetylase activity of	is not required for					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_1_118_s_36	12147236	By using a acetylase defective mutant of CBP (L1690K/C1691L), we have found that the acetylase activity of CBP is not required for stimulation of p53 DNA binding (unpublished data).	transcription
73035	1	336336	7	NULL	NULL	0	NULL	p53	GP		associates with					chromatin	Chromosome				NULL		0	NULL	NULL	NULL	gw60_cell_107_7_815_s_49	11779456	Roles of Acetylation in Transcriptional Regulation  by p53 Association of p53 (blue spheres) with chromatin  is not affected by its state of  acetylation, but p53-dependent alterations in chromatin structure by  histone acetylation and subsequent recruitment of the  transcriptional machinery (general transcription factors, mediator and RNA  polymerase II) are facilitated by interactions with acetylases, and  possibly by acetylation of p53 itself (acetyl  groups on p53 and histones are indicated  by red circles).	transcription
73036	2	336336	7	NULL	NULL	0	NULL	statement 1	Process		is not affected by					p53	GP	acetylation of			NULL		0	NULL	NULL	NULL	gw60_cell_107_7_815_s_49	11779456	Roles of Acetylation in Transcriptional Regulation  by p53 Association of p53 (blue spheres) with chromatin  is not affected by its state of  acetylation, but p53-dependent alterations in chromatin structure by  histone acetylation and subsequent recruitment of the  transcriptional machinery (general transcription factors, mediator and RNA  polymerase II) are facilitated by interactions with acetylases, and  possibly by acetylation of p53 itself (acetyl  groups on p53 and histones are indicated  by red circles).	transcription
73037	3	336336	7	NULL	NULL	0	NULL	chromatin structure	Chromosome	alterations in	depends on					p53	GP				NULL		0	NULL	NULL	NULL	gw60_cell_107_7_815_s_49	11779456	Roles of Acetylation in Transcriptional Regulation  by p53 Association of p53 (blue spheres) with chromatin  is not affected by its state of  acetylation, but p53-dependent alterations in chromatin structure by  histone acetylation and subsequent recruitment of the  transcriptional machinery (general transcription factors, mediator and RNA  polymerase II) are facilitated by interactions with acetylases, and  possibly by acetylation of p53 itself (acetyl  groups on p53 and histones are indicated  by red circles).	transcription
73038	4	336336	7	NULL	NULL	0	NULL	statement 3	Process		occur by					histone	GP	acetylation of			NULL		0	NULL	NULL	NULL	gw60_cell_107_7_815_s_49	11779456	Roles of Acetylation in Transcriptional Regulation  by p53 Association of p53 (blue spheres) with chromatin  is not affected by its state of  acetylation, but p53-dependent alterations in chromatin structure by  histone acetylation and subsequent recruitment of the  transcriptional machinery (general transcription factors, mediator and RNA  polymerase II) are facilitated by interactions with acetylases, and  possibly by acetylation of p53 itself (acetyl  groups on p53 and histones are indicated  by red circles).	transcription
73039	5	336336	7	NULL	NULL	0	NULL	statement 4	Process		followed by					transcription factors	GP	subsequent recruitment of			NULL		0	NULL	NULL	NULL	gw60_cell_107_7_815_s_49	11779456	Roles of Acetylation in Transcriptional Regulation  by p53 Association of p53 (blue spheres) with chromatin  is not affected by its state of  acetylation, but p53-dependent alterations in chromatin structure by  histone acetylation and subsequent recruitment of the  transcriptional machinery (general transcription factors, mediator and RNA  polymerase II) are facilitated by interactions with acetylases, and  possibly by acetylation of p53 itself (acetyl  groups on p53 and histones are indicated  by red circles).	transcription
73040	6	336336	7	NULL	NULL	0	NULL	statement 4	Process		followed by					RNA polymerase II	GP	subsequent recruitment of			NULL		0	NULL	NULL	NULL	gw60_cell_107_7_815_s_49	11779456	Roles of Acetylation in Transcriptional Regulation  by p53 Association of p53 (blue spheres) with chromatin  is not affected by its state of  acetylation, but p53-dependent alterations in chromatin structure by  histone acetylation and subsequent recruitment of the  transcriptional machinery (general transcription factors, mediator and RNA  polymerase II) are facilitated by interactions with acetylases, and  possibly by acetylation of p53 itself (acetyl  groups on p53 and histones are indicated  by red circles).	transcription
73041	7	336336	7	NULL	NULL	0	NULL	statement 5	Process		facilitated by					acetylases	GP	interactions with			NULL		0	NULL	NULL	NULL	gw60_cell_107_7_815_s_49	11779456	Roles of Acetylation in Transcriptional Regulation  by p53 Association of p53 (blue spheres) with chromatin  is not affected by its state of  acetylation, but p53-dependent alterations in chromatin structure by  histone acetylation and subsequent recruitment of the  transcriptional machinery (general transcription factors, mediator and RNA  polymerase II) are facilitated by interactions with acetylases, and  possibly by acetylation of p53 itself (acetyl  groups on p53 and histones are indicated  by red circles).	transcription
73042	8	336336	7	NULL	NULL	0	NULL	statement 6	Process		facilitated by					acetylases	GP	interactions with			NULL		0	NULL	NULL	NULL	gw60_cell_107_7_815_s_49	11779456	Roles of Acetylation in Transcriptional Regulation  by p53 Association of p53 (blue spheres) with chromatin  is not affected by its state of  acetylation, but p53-dependent alterations in chromatin structure by  histone acetylation and subsequent recruitment of the  transcriptional machinery (general transcription factors, mediator and RNA  polymerase II) are facilitated by interactions with acetylases, and  possibly by acetylation of p53 itself (acetyl  groups on p53 and histones are indicated  by red circles).	transcription
73043	9	336336	7	NULL	NULL	0	NULL	statement 5	Process		facilitated by					p53	GP	acetylation of			NULL		0	NULL	NULL	NULL	gw60_cell_107_7_815_s_49	11779456	Roles of Acetylation in Transcriptional Regulation  by p53 Association of p53 (blue spheres) with chromatin  is not affected by its state of  acetylation, but p53-dependent alterations in chromatin structure by  histone acetylation and subsequent recruitment of the  transcriptional machinery (general transcription factors, mediator and RNA  polymerase II) are facilitated by interactions with acetylases, and  possibly by acetylation of p53 itself (acetyl  groups on p53 and histones are indicated  by red circles).	transcription
73044	10	336336	7	NULL	NULL	0	NULL	statement 6	Process		facilitated by					p53	GP	acetylation of			NULL		0	NULL	NULL	NULL	gw60_cell_107_7_815_s_49	11779456	Roles of Acetylation in Transcriptional Regulation  by p53 Association of p53 (blue spheres) with chromatin  is not affected by its state of  acetylation, but p53-dependent alterations in chromatin structure by  histone acetylation and subsequent recruitment of the  transcriptional machinery (general transcription factors, mediator and RNA  polymerase II) are facilitated by interactions with acetylases, and  possibly by acetylation of p53 itself (acetyl  groups on p53 and histones are indicated  by red circles).	transcription
73045	1	336337	7	NULL	NULL	NULL	NULL	MageA2	GP		down-regulate					p53	GP	mutant;;nonacetylable;;transcriptional activity of 	9KR		NULL		NULL	NULL	NULL	NULL	gw70_pnas_103_30_11160_s_110	16847267	In fact, MageA2 was able to down-regulate the transcriptional activity of the nonacetylable p53 mutant, p539KR ( ), both alone or when cotransfected with the histone acetyl transferase p300 (Fig. 7  C and  D), strongly suggesting that histone hypoacetylation could represent the main mechanism used by MageA2 for targeting p53 activity.	transcription
73046	2	336337	7	NULL	NULL	0	NULL	MageA2	GP		target					p53	GP	activity of			NULL		0	NULL	NULL	NULL	gw70_pnas_103_30_11160_s_110	16847267	In fact, MageA2 was able to down-regulate the transcriptional activity of the nonacetylable p53 mutant, p539KR ( ), both alone or when cotransfected with the histone acetyl transferase p300 (Fig. 7  C and  D), strongly suggesting that histone hypoacetylation could represent the main mechanism used by MageA2 for targeting p53 activity.	transcription
73047	3	336337	7	NULL	NULL	0	NULL	histone	GP	hypoacetylation of	mechanism for					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_103_30_11160_s_110	16847267	In fact, MageA2 was able to down-regulate the transcriptional activity of the nonacetylable p53 mutant, p539KR ( ), both alone or when cotransfected with the histone acetyl transferase p300 (Fig. 7  C and  D), strongly suggesting that histone hypoacetylation could represent the main mechanism used by MageA2 for targeting p53 activity.	transcription
73048	4	336337	7	NULL	NULL	0	NULL	statement 1	Process		suggest		strongly			statement 3	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_103_30_11160_s_110	16847267	In fact, MageA2 was able to down-regulate the transcriptional activity of the nonacetylable p53 mutant, p539KR ( ), both alone or when cotransfected with the histone acetyl transferase p300 (Fig. 7  C and  D), strongly suggesting that histone hypoacetylation could represent the main mechanism used by MageA2 for targeting p53 activity.	transcription
73050	1	336338	7	NULL	NULL	0	NULL	CBP/p300	GP		shows					FAT activity	Process				NULL		0	NULL	NULL	NULL	gw60_cell_107_2_137_s_16	11672522	Significantly, the  observation of functional synergism between p53 and  CBP/p300 together with its intrinsic HAT activity  led to the discovery of an FAT  (transcriptional  factor  acetyl- transferase) activity of CBP/p300 on p53; this  finding also predicted that acetylation may represent  a general functional modification for nonhistone proteins  in vivo (Gu and Roeder, 1997   ).	transcription
73051	2	336338	7	NULL	NULL	0	NULL	statement 1	Process		occur on					p53	GP				NULL		0	NULL	NULL	NULL	gw60_cell_107_2_137_s_16	11672522	Significantly, the  observation of functional synergism between p53 and  CBP/p300 together with its intrinsic HAT activity  led to the discovery of an FAT  (transcriptional  factor  acetyl- transferase) activity of CBP/p300 on p53; this  finding also predicted that acetylation may represent  a general functional modification for nonhistone proteins  in vivo (Gu and Roeder, 1997   ).	transcription
73052	3	336338	7	NULL	NULL	0	NULL	acetylation	Process		represent		may			nonhistone proteins	GP	functional modification for			NULL	in vivo	0	NULL	NULL	NULL	gw60_cell_107_2_137_s_16	11672522	Significantly, the  observation of functional synergism between p53 and  CBP/p300 together with its intrinsic HAT activity  led to the discovery of an FAT  (transcriptional  factor  acetyl- transferase) activity of CBP/p300 on p53; this  finding also predicted that acetylation may represent  a general functional modification for nonhistone proteins  in vivo (Gu and Roeder, 1997   ).	transcription
73053	4	336338	7	NULL	NULL	0	NULL	statement 2	Process		predicts					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_cell_107_2_137_s_16	11672522	Significantly, the  observation of functional synergism between p53 and  CBP/p300 together with its intrinsic HAT activity  led to the discovery of an FAT  (transcriptional  factor  acetyl- transferase) activity of CBP/p300 on p53; this  finding also predicted that acetylation may represent  a general functional modification for nonhistone proteins  in vivo (Gu and Roeder, 1997   ).	transcription
73054	5	336338	7	NULL	NULL	0	NULL	FAT	GP		is					transcriptional factor acetyl- transferase	GP				NULL		0	NULL	NULL	NULL	gw60_cell_107_2_137_s_16	11672522	Significantly, the  observation of functional synergism between p53 and  CBP/p300 together with its intrinsic HAT activity  led to the discovery of an FAT  (transcriptional  factor  acetyl- transferase) activity of CBP/p300 on p53; this  finding also predicted that acetylation may represent  a general functional modification for nonhistone proteins  in vivo (Gu and Roeder, 1997   ).	transcription
73055	1	336339	7	NULL	NULL	0	NULL	Acetyl-CoA	Chemical		stabilizes					p300.p53AC complex	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_15_13431_s_239	12499368	Acetyl-CoA Stabilizes the p300.p53AC Complex--  With the  DNA-dependent p53 acetylation assay biochemically characterized, we could finally access the role of the phospho-Ser20 peptide-binding domains of p300 to both DNA-dependent p53 acetylation and DNA-independent histone acetylation (Fig.  8).	transcription
73056	2	336339	7	NULL	NULL	0	NULL	p53	GP	acetylation of	depends on					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_15_13431_s_239	12499368	Acetyl-CoA Stabilizes the p300.p53AC Complex--  With the  DNA-dependent p53 acetylation assay biochemically characterized, we could finally access the role of the phospho-Ser20 peptide-binding domains of p300 to both DNA-dependent p53 acetylation and DNA-independent histone acetylation (Fig.  8).	transcription
73057	3	336339	7	NULL	NULL	0	NULL	histone	GP	acetylation of	independent of					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_15_13431_s_239	12499368	Acetyl-CoA Stabilizes the p300.p53AC Complex--  With the  DNA-dependent p53 acetylation assay biochemically characterized, we could finally access the role of the phospho-Ser20 peptide-binding domains of p300 to both DNA-dependent p53 acetylation and DNA-independent histone acetylation (Fig.  8).	transcription
73058	1	336340	7	NULL	NULL	0	NULL	 p300 protein	GP		bind		stably			p53 protein	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_15_13431_s_274	12499368	The amount of p300 protein stably bound to p53 protein: ( /+)-acetyl-CoA, ( /+)-NS-DNA, or  ( /+)-pG-DNA was determined using an antibody to p300 and quantitated as p300 bound/total p53 using enhanced chemiluminescence expressed as relative light units ( RLU).	transcription
73106	1	336342	7	NULL	NULL	0	NULL	MDM2	GP		degrade					p53	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_9_7453_s_28	12493762	However, it is unclear whether p300 requires its acetylase activity to assist MDM2 in degrading p53.	transcription
73107	2	336342	7	NULL	NULL	NULL	NULL	p300	GP		activates 					acetylase	GP				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_278_9_7453_s_28	12493762	However, it is unclear whether p300 requires its acetylase activity to assist MDM2 in degrading p53.	transcription
73108	1	336343	7	NULL	NULL	0	NULL	CBP/p300	GP		acetylate					p53	GP				NULL		0	NULL	NULL	NULL	gw70_embo_25_8_1680_s_251	16601686	Alternatively, Tip60 can affect  the function of other HATs, such as CBP/p300, which are known to acetylate p53 ( ).	transcription
73109	2	336343	7	NULL	NULL	0	NULL	Tip60	GP		affect					CBP/p300 	GP	function of			NULL		0	NULL	NULL	NULL	gw70_embo_25_8_1680_s_251	16601686	Alternatively, Tip60 can affect  the function of other HATs, such as CBP/p300, which are known to acetylate p53 ( ).	transcription
73110	3	336343	7	NULL	NULL	0	NULL	CBP/p300	GP		is a type of					HAT	GP				NULL		0	NULL	NULL	NULL	gw70_embo_25_8_1680_s_251	16601686	Alternatively, Tip60 can affect  the function of other HATs, such as CBP/p300, which are known to acetylate p53 ( ).	transcription
73111	1	336344	7	NULL	NULL	0	NULL	p53	GP		interacts with					p300/CBP	GP				NULL		0	NULL	NULL	NULL	gw70_embo_24_14_2634_s_198	16001085	Moreover,  like p53, Tip60 was found to interact with p300/CBP, which could also acetylate the  protein on two specific lysines.	transcription
73112	2	336344	7	NULL	NULL	0	NULL	 Tip60	GP		interacts with					p300/CBP	GP				NULL		0	NULL	NULL	NULL	gw70_embo_24_14_2634_s_198	16001085	Moreover,  like p53, Tip60 was found to interact with p300/CBP, which could also acetylate the  protein on two specific lysines.	transcription
73113	3	336344	7	NULL	NULL	0	NULL	p300/CBP	GP		acetylate					Tip60	GP		two specific lysine		NULL		0	NULL	NULL	NULL	gw70_embo_24_14_2634_s_198	16001085	Moreover,  like p53, Tip60 was found to interact with p300/CBP, which could also acetylate the  protein on two specific lysines.	transcription
73114	4	336344	7	NULL	NULL	0	NULL	statement 1	Process		is similar to					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_embo_24_14_2634_s_198	16001085	Moreover,  like p53, Tip60 was found to interact with p300/CBP, which could also acetylate the  protein on two specific lysines.	transcription
73115	1	336345	7	NULL	NULL	0	NULL	p53	GP		bind					CBP	GP				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_27_4_673_s_77	16308315	It also enables the binding of p53 to CBP, p300 and p/CAF (   -  ), which acetylate it at certain specific lysine residues ( , ).	transcription
73116	2	336345	7	NULL	NULL	0	NULL	p53	GP		bind					p300	GP				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_27_4_673_s_77	16308315	It also enables the binding of p53 to CBP, p300 and p/CAF (   -  ), which acetylate it at certain specific lysine residues ( , ).	transcription
73117	3	336345	7	NULL	NULL	0	NULL	p53	GP		bind					p/CAF	GP				NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_27_4_673_s_77	16308315	It also enables the binding of p53 to CBP, p300 and p/CAF (   -  ), which acetylate it at certain specific lysine residues ( , ).	transcription
73118	4	336345	7	NULL	NULL	NULL	NULL	CBP	GP		acetylate					p53			lysine residue		NULL		NULL	NULL	NULL	NULL	gw70_carcinogenesis_27_4_673_s_77	16308315	It also enables the binding of p53 to CBP, p300 and p/CAF (   -  ), which acetylate it at certain specific lysine residues ( , ).	transcription
73119	5	336345	7	NULL	NULL	0	NULL	p300	GP		acetylate					p53	GP		lysine residue		NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_27_4_673_s_77	16308315	It also enables the binding of p53 to CBP, p300 and p/CAF (   -  ), which acetylate it at certain specific lysine residues ( , ).	transcription
73120	6	336345	7	NULL	NULL	0	NULL	p/CAF	GP		acetylate					p53	GP		lysine residue		NULL		0	NULL	NULL	NULL	gw70_carcinogenesis_27_4_673_s_77	16308315	It also enables the binding of p53 to CBP, p300 and p/CAF (   -  ), which acetylate it at certain specific lysine residues ( , ).	transcription
73159	1	336346	7	NULL	NULL	0	NULL	p300	GP		acetylate					histones	GP				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_67_0_545_s_310	9759497	For example, in addition to histones, p300 will acetylate the tumor suppressor  protein, p53, enhancing its in vitro DNA-binding activity ( 202).	transcription
73160	2	336346	7	NULL	NULL	0	NULL	p300	GP		acetylate					p53	GP				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_67_0_545_s_310	9759497	For example, in addition to histones, p300 will acetylate the tumor suppressor  protein, p53, enhancing its in vitro DNA-binding activity ( 202).	transcription
73161	3	336346	7	NULL	NULL	0	NULL	statement 2	Process		enhance					DNA-binding activity	Process				NULL	in vitro	0	NULL	NULL	NULL	gw70_annurevbiochem_67_0_545_s_310	9759497	For example, in addition to histones, p300 will acetylate the tumor suppressor  protein, p53, enhancing its in vitro DNA-binding activity ( 202).	transcription
73162	4	336346	7	NULL	NULL	0	NULL	p53	GP		is a type of					tumor suppressor protein	GP				NULL		0	NULL	NULL	NULL	gw70_annurevbiochem_67_0_545_s_310	9759497	For example, in addition to histones, p300 will acetylate the tumor suppressor  protein, p53, enhancing its in vitro DNA-binding activity ( 202).	transcription
73163	1	336347	7	NULL	NULL	0	NULL	p300-deficient cells	Cell		fails to		fully			p53	GP	acetylate			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_15_6639_s_316	16024799	Hence, p300-deficient cells fail to fully acetylate p53 and do not transactivate p21 or undergo G1/S arrest after UV irradiation ( ).	transcription
73164	2	336347	7	NULL	NULL	NULL	NULL	 p300-deficient cells	Cell		does not transactivate					p21	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_15_6639_s_316	16024799	Hence, p300-deficient cells fail to fully acetylate p53 and do not transactivate p21 or undergo G1/S arrest after UV irradiation ( ).	transcription
73165	3	336347	7	NULL	NULL	0	NULL	p300-deficient cells	Cell		does not undergo					G1/S arrest	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_15_6639_s_316	16024799	Hence, p300-deficient cells fail to fully acetylate p53 and do not transactivate p21 or undergo G1/S arrest after UV irradiation ( ).	transcription
73166	4	336347	7	NULL	NULL	0	NULL	statement 3	Process		occur after					UV irradiation	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_15_6639_s_316	16024799	Hence, p300-deficient cells fail to fully acetylate p53 and do not transactivate p21 or undergo G1/S arrest after UV irradiation ( ).	transcription
73167	1	336348	7	NULL	NULL	0	NULL	p300	GP		does not acetylate					p53 tetramers	GP	native			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_2	14612423	The transcription coactivator p300 cannot acetylate native p53 tetramers, thus revealing intrinsic conformational constraints on p300-catalyzed acetylation.	transcription
73168	2	336348	7	NULL	NULL	0	NULL	p300	GP		catalyze					acetylation	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_2	14612423	The transcription coactivator p300 cannot acetylate native p53 tetramers, thus revealing intrinsic conformational constraints on p300-catalyzed acetylation.	transcription
73169	3	336348	7	NULL	NULL	0	NULL	statement 1	Process		reveal					statement 2	Process	intrinsic conformational constraints			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_2	14612423	The transcription coactivator p300 cannot acetylate native p53 tetramers, thus revealing intrinsic conformational constraints on p300-catalyzed acetylation.	transcription
73170	4	336348	7	NULL	NULL	0	NULL	p300	GP		is a type of					 transcription coactivator	GP				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_2	14612423	The transcription coactivator p300 cannot acetylate native p53 tetramers, thus revealing intrinsic conformational constraints on p300-catalyzed acetylation.	transcription
73171	1	336349	7	NULL	NULL	NULL	NULL	p53	GP		recruit					p300	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_1_57_s_237	11511360	Particularly whether p53 recruits p300 to acetylate nucleosomal histones within the p21 promoter.	transcription
73172	2	336349	7	NULL	NULL	0	NULL	statement 1	Process		acetylate					nucleosomal histones	GP				NULL		0	NULL	NULL	NULL	gw60_molcell_8_1_57_s_237	11511360	Particularly whether p53 recruits p300 to acetylate nucleosomal histones within the p21 promoter.	transcription
73173	3	336349	7	NULL	NULL	0	NULL	statement 2	Process		occur within					p21	GP			promoter	NULL		0	NULL	NULL	NULL	gw60_molcell_8_1_57_s_237	11511360	Particularly whether p53 recruits p300 to acetylate nucleosomal histones within the p21 promoter.	transcription
73174	1	336350	7	NULL	NULL	0	NULL	PCAF 	GP		acetylate					p53	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_12_8136_s_28	10567539	PCAF can also acetylate p53, but at a different site ( 45), and chromosomal protein HMG-17 ( 32).	transcription
73175	2	336350	7	NULL	NULL	0	NULL	PCAF	GP		acetylate					HMG-17	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_12_8136_s_28	10567539	PCAF can also acetylate p53, but at a different site ( 45), and chromosomal protein HMG-17 ( 32).	transcription
73176	3	336350	7	NULL	NULL	0	NULL	HMG-17	GP		is a type of					chromosomal protein	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_12_8136_s_28	10567539	PCAF can also acetylate p53, but at a different site ( 45), and chromosomal protein HMG-17 ( 32).	transcription
73177	4	336350	7	NULL	NULL	0	NULL	statement 1	Process	binding site of	is different from					statement 2	Process	binding site of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_12_8136_s_28	10567539	PCAF can also acetylate p53, but at a different site ( 45), and chromosomal protein HMG-17 ( 32).	transcription
73178	1	336351	7	NULL	NULL	0	NULL	p300	GP	HAT activity of	acetylate					p53	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6367_s_359	10454583	The HAT activity of p300 can acetylate p53, increasing its sequence-specific DNA binding activity ( 13).	transcription
73179	2	336351	7	NULL	NULL	NULL	NULL	p53	GP		bind		sequence-specific			DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_19_9_6367_s_359	10454583	The HAT activity of p300 can acetylate p53, increasing its sequence-specific DNA binding activity ( 13).	transcription
73180	3	336351	7	NULL	NULL	0	NULL	statement 1	Process		increase					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_9_6367_s_359	10454583	The HAT activity of p300 can acetylate p53, increasing its sequence-specific DNA binding activity ( 13).	transcription
73181	1	336352	7	NULL	NULL	0	NULL	CBP/p300	GP		acetylate					p53	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_20_16804_s_26	11279157	For example, CBP/p300 can acetylate p53, resulting in an enhancement of its DNA binding activity.	transcription
73182	2	336352	7	NULL	NULL	0	NULL	p53	GP		bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_20_16804_s_26	11279157	For example, CBP/p300 can acetylate p53, resulting in an enhancement of its DNA binding activity.	transcription
73183	3	336352	7	NULL	NULL	0	NULL	statement 1	Process		enhance					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_20_16804_s_26	11279157	For example, CBP/p300 can acetylate p53, resulting in an enhancement of its DNA binding activity.	transcription
73184	1	336353	7	NULL	NULL	0	NULL	stress	Process		activate					p53	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_50566_s_428	15364927	It is well known that various types of stress activate p53 through inducing phosphorylation of p53 by a number of kinases and acetylation of p53 by acetylases p300 and PCAF ( ).	transcription
73185	3	336353	7	NULL	NULL	NULL	NULL	statement 1	Process		through					statement 2	GP				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_48_50566_s_428	15364927	It is well known that various types of stress activate p53 through inducing phosphorylation of p53 by a number of kinases and acetylation of p53 by acetylases p300 and PCAF ( ).	transcription
73186	2	336353	7	NULL	NULL	NULL	NULL	kinases	GP		induce					p53	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_48_50566_s_428	15364927	It is well known that various types of stress activate p53 through inducing phosphorylation of p53 by a number of kinases and acetylation of p53 by acetylases p300 and PCAF ( ).	transcription
73187	4	336353	7	NULL	NULL	0	NULL	p300	GP		induce					p53	GP	acetylation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_50566_s_428	15364927	It is well known that various types of stress activate p53 through inducing phosphorylation of p53 by a number of kinases and acetylation of p53 by acetylases p300 and PCAF ( ).	transcription
73188	5	336353	7	NULL	NULL	0	NULL	PCAF	GP		induce					p53	GP	acetylation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_50566_s_428	15364927	It is well known that various types of stress activate p53 through inducing phosphorylation of p53 by a number of kinases and acetylation of p53 by acetylases p300 and PCAF ( ).	transcription
73189	6	336353	7	NULL	NULL	0	NULL	p300	GP		is a type of					acetylases	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_50566_s_428	15364927	It is well known that various types of stress activate p53 through inducing phosphorylation of p53 by a number of kinases and acetylation of p53 by acetylases p300 and PCAF ( ).	transcription
73190	7	336353	7	NULL	NULL	0	NULL	PCAF	GP		is a type of					acetylases	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_50566_s_428	15364927	It is well known that various types of stress activate p53 through inducing phosphorylation of p53 by a number of kinases and acetylation of p53 by acetylases p300 and PCAF ( ).	transcription
73191	8	336353	7	NULL	NULL	0	NULL	statement 1	Process		through					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_50566_s_428	15364927	It is well known that various types of stress activate p53 through inducing phosphorylation of p53 by a number of kinases and acetylation of p53 by acetylases p300 and PCAF ( ).	transcription
73192	9	336353	7	NULL	NULL	0	NULL	statement 1	Process		through					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_50566_s_428	15364927	It is well known that various types of stress activate p53 through inducing phosphorylation of p53 by a number of kinases and acetylation of p53 by acetylases p300 and PCAF ( ).	transcription
73193	1	336354	7	NULL	NULL	0	NULL	 p300	GP		acetylates					p53	GP				NULL	in vivo	0	NULL	NULL	NULL	gw60_embo_20_6_1331_s_50	11250899	We also establish that,  in vivo, p300 and CBP can function as p53 acetylases and positively regulate p53 acetylation status, while MDM2 suppresses p53 acetylation.	transcription
73194	2	336354	7	NULL	NULL	NULL	NULL	CBP 	GP		acetylates					p53	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_embo_20_6_1331_s_50	11250899	We also establish that,  in vivo, p300 and CBP can function as p53 acetylases and positively regulate p53 acetylation status, while MDM2 suppresses p53 acetylation.	transcription
73195	3	336354	7	NULL	NULL	0	NULL	statement 1	Process		regulates		positively			p53	GP				NULL		0	NULL	NULL	NULL	gw60_embo_20_6_1331_s_50	11250899	We also establish that,  in vivo, p300 and CBP can function as p53 acetylases and positively regulate p53 acetylation status, while MDM2 suppresses p53 acetylation.	transcription
73196	4	336354	7	NULL	NULL	0	NULL	statement 2	Process		regulates		positively			p53	GP				NULL		0	NULL	NULL	NULL	gw60_embo_20_6_1331_s_50	11250899	We also establish that,  in vivo, p300 and CBP can function as p53 acetylases and positively regulate p53 acetylation status, while MDM2 suppresses p53 acetylation.	transcription
73197	5	336354	7	NULL	NULL	0	NULL	MDM2	GP		suppress					p53	GP	acetylation of			NULL		0	NULL	NULL	NULL	gw60_embo_20_6_1331_s_50	11250899	We also establish that,  in vivo, p300 and CBP can function as p53 acetylases and positively regulate p53 acetylation status, while MDM2 suppresses p53 acetylation.	transcription
73198	1	336355	7	NULL	NULL	NULL	NULL	PCAF	GP		interacts with		physically			p53	GP				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5540_s_8	10891493	We further show that the E1B 55-kDa protein interferes with the physical interaction between PCAF and p53, suggesting that the E1B 55-kDa protein inhibits PCAF acetylase function on p53 by preventing enzyme-substrate interaction.	transcription
73199	2	336355	7	NULL	NULL	0	NULL	 E1B 55-kDa protein	GP		interferes with					statement 1	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_15_5540_s_8	10891493	We further show that the E1B 55-kDa protein interferes with the physical interaction between PCAF and p53, suggesting that the E1B 55-kDa protein inhibits PCAF acetylase function on p53 by preventing enzyme-substrate interaction.	transcription
73200	3	336355	7	NULL	NULL	0	NULL	PCAF	GP		acetylates					p53	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_15_5540_s_8	10891493	We further show that the E1B 55-kDa protein interferes with the physical interaction between PCAF and p53, suggesting that the E1B 55-kDa protein inhibits PCAF acetylase function on p53 by preventing enzyme-substrate interaction.	transcription
73201	4	336355	7	NULL	NULL	0	NULL	E1B 55-kDa protein 	GP		inhibits					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_15_5540_s_8	10891493	We further show that the E1B 55-kDa protein interferes with the physical interaction between PCAF and p53, suggesting that the E1B 55-kDa protein inhibits PCAF acetylase function on p53 by preventing enzyme-substrate interaction.	transcription
73202	1	336356	7	NULL	NULL	0	NULL	p300	GP		activates					acetylase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_49_45928_s_138	11591713	Since the acetylase activity of p300 is required for its stabilization of MDM2 but not for stabilization of p53, one would predict that the p300DY mutant's ability to stabilize p53 would not be affected by MDM2 expression.	transcription
73203	2	336356	7	NULL	NULL	0	NULL	statement 1	Process		required for					MDM2	GP	stabilization of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_49_45928_s_138	11591713	Since the acetylase activity of p300 is required for its stabilization of MDM2 but not for stabilization of p53, one would predict that the p300DY mutant's ability to stabilize p53 would not be affected by MDM2 expression.	transcription
73204	3	336356	7	NULL	NULL	NULL	NULL	statement 1	Process		is not required for					p53	GP	stabilization of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_276_49_45928_s_138	11591713	Since the acetylase activity of p300 is required for its stabilization of MDM2 but not for stabilization of p53, one would predict that the p300DY mutant's ability to stabilize p53 would not be affected by MDM2 expression.	transcription
73205	4	336356	7	NULL	NULL	0	NULL	p300	GP	mutant	stabilize			DY		p53	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_49_45928_s_138	11591713	Since the acetylase activity of p300 is required for its stabilization of MDM2 but not for stabilization of p53, one would predict that the p300DY mutant's ability to stabilize p53 would not be affected by MDM2 expression.	transcription
73206	5	336356	7	NULL	NULL	0	NULL	MDM2	GP	expression of	does not affect					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_49_45928_s_138	11591713	Since the acetylase activity of p300 is required for its stabilization of MDM2 but not for stabilization of p53, one would predict that the p300DY mutant's ability to stabilize p53 would not be affected by MDM2 expression.	transcription
73207	1	336357	7	NULL	NULL	NULL	NULL	p300	GP		acetylates					p53	GP		N terminus		NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_24_23_10366_s_289	15542844	Other molecules that interact with the p53 N terminus, such as the transcriptional coactivator p300 that acetylates p53 ( ), and the MdmX protein ( ,  ) can also contribute to p53 stabilization.	transcription
73208	2	336357	7	NULL	NULL	0	NULL	p300	GP		acetylates					MdmX protein 	GP				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_23_10366_s_289	15542844	Other molecules that interact with the p53 N terminus, such as the transcriptional coactivator p300 that acetylates p53 ( ), and the MdmX protein ( ,  ) can also contribute to p53 stabilization.	transcription
73209	3	336357	7	NULL	NULL	0	NULL	p300	GP		contribute to					p53	GP	stabilization of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_23_10366_s_289	15542844	Other molecules that interact with the p53 N terminus, such as the transcriptional coactivator p300 that acetylates p53 ( ), and the MdmX protein ( ,  ) can also contribute to p53 stabilization.	transcription
73210	4	336357	7	NULL	NULL	0	NULL	p300	GP		is a type of					transcriptional coactivator 	GP				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_23_10366_s_289	15542844	Other molecules that interact with the p53 N terminus, such as the transcriptional coactivator p300 that acetylates p53 ( ), and the MdmX protein ( ,  ) can also contribute to p53 stabilization.	transcription
73211	1	336358	7	NULL	NULL	0	NULL	p53	GP		interacts with					p300/CBP	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1602_1_47_s_122	11960694	N-terminal phosphorylation also enhances interactions of p53 with transcriptional co-activators like p300/CBP, which can acetylate residues in the C-terminus and promote p53's transcriptional activity.	transcription
73212	2	336358	7	NULL	NULL	0	NULL	p300/CBP	GP		acetylate					p53	GP		C-terminus		NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1602_1_47_s_122	11960694	N-terminal phosphorylation also enhances interactions of p53 with transcriptional co-activators like p300/CBP, which can acetylate residues in the C-terminus and promote p53's transcriptional activity.	transcription
73213	3	336358	7	NULL	NULL	0	NULL	statement 2	Process		promote					p53	GP	transcriptional activity of			NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1602_1_47_s_122	11960694	N-terminal phosphorylation also enhances interactions of p53 with transcriptional co-activators like p300/CBP, which can acetylate residues in the C-terminus and promote p53's transcriptional activity.	transcription
73214	4	336358	7	NULL	NULL	NULL	NULL	p53		phosphorylation 	enhance			N-terminal		statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1602_1_47_s_122	11960694	N-terminal phosphorylation also enhances interactions of p53 with transcriptional co-activators like p300/CBP, which can acetylate residues in the C-terminus and promote p53's transcriptional activity.	transcription
73215	5	336358	7	NULL	NULL	0	NULL	p300/CBP	GP		is a type of					transcriptional co-activator	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1602_1_47_s_122	11960694	N-terminal phosphorylation also enhances interactions of p53 with transcriptional co-activators like p300/CBP, which can acetylate residues in the C-terminus and promote p53's transcriptional activity.	transcription
73216	1	336359	7	NULL	NULL	0	NULL	PCAF	GP		acetylate		specifically			p53	GP		lysine 320		NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_34_30838_s_17	12068014	Although less studied, the  p300/ CBP- associated  factor (PCAF) has also been shown to specifically acetylate the lysine 320 of p53, leading to the enhancement of the sequence-specific DNA binding activity of p53  in vitro ( 13).	transcription
73217	2	336359	7	NULL	NULL	0	NULL	p53	GP		bind		sequence-specific			DNA	NucleicAcid				NULL	in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_277_34_30838_s_17	12068014	Although less studied, the  p300/ CBP- associated  factor (PCAF) has also been shown to specifically acetylate the lysine 320 of p53, leading to the enhancement of the sequence-specific DNA binding activity of p53  in vitro ( 13).	transcription
73218	3	336359	7	NULL	NULL	0	NULL	statement 1	Process		enhance					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_34_30838_s_17	12068014	Although less studied, the  p300/ CBP- associated  factor (PCAF) has also been shown to specifically acetylate the lysine 320 of p53, leading to the enhancement of the sequence-specific DNA binding activity of p53  in vitro ( 13).	transcription
73219	4	336359	7	NULL	NULL	0	NULL	PCAF	GP		is					p300/ CBP- associated factor	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_277_34_30838_s_17	12068014	Although less studied, the  p300/ CBP- associated  factor (PCAF) has also been shown to specifically acetylate the lysine 320 of p53, leading to the enhancement of the sequence-specific DNA binding activity of p53  in vitro ( 13).	transcription
73220	1	336360	7	NULL	NULL	0	NULL	TRRAP	GP		bind					p53	GP	acetylated			NULL	in vitro	0	NULL	NULL	NULL	gw60_molcell_8_6_1243_s_241	11779500	Binding of TRRAP and hGcn5 to Acetylated p53 In Vitro	transcription
73221	2	336360	7	NULL	NULL	0	NULL	hGcn5	GP		bind					p53	GP	acetylated			NULL	in vitro	0	NULL	NULL	NULL	gw60_molcell_8_6_1243_s_241	11779500	Binding of TRRAP and hGcn5 to Acetylated p53 In Vitro	transcription
73222	1	336361	7	NULL	NULL	0	NULL	Sir2 enzyme 	GP		bind					p53 peptide	GP	acetylated			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_23_9_3173_s_447	12697818	Structure of a Sir2 enzyme bound to an acetylated p53 peptide.	transcription
73223	1	336362	7	NULL	NULL	0	NULL	p300	GP		activates					acetylase	GP				NULL	in vitro	0	NULL	NULL	NULL	gw60_jbiolchem_276_1_48_s_168	11076933	First of all, p73alpha was a considerably poor substrate for the acetylase activity of p300  in vitro, in contrast with p53, which is acetylated by p300 in response to DNA damage ( 12,  13).	transcription
73224	2	336362	7	NULL	NULL	0	NULL	p73alpha	GP		poor substrate for					statement 1	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_48_s_168	11076933	First of all, p73alpha was a considerably poor substrate for the acetylase activity of p300  in vitro, in contrast with p53, which is acetylated by p300 in response to DNA damage ( 12,  13).	transcription
73225	3	336362	7	NULL	NULL	0	NULL	p300	GP		acetylates					p53	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_48_s_168	11076933	First of all, p73alpha was a considerably poor substrate for the acetylase activity of p300  in vitro, in contrast with p53, which is acetylated by p300 in response to DNA damage ( 12,  13).	transcription
73226	4	336362	7	NULL	NULL	0	NULL	statement 3	Process		in response to					DNA damage	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_48_s_168	11076933	First of all, p73alpha was a considerably poor substrate for the acetylase activity of p300  in vitro, in contrast with p53, which is acetylated by p300 in response to DNA damage ( 12,  13).	transcription
73227	5	336362	7	NULL	NULL	0	NULL	statement 2	Process		in contrast with					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_276_1_48_s_168	11076933	First of all, p73alpha was a considerably poor substrate for the acetylase activity of p300  in vitro, in contrast with p53, which is acetylated by p300 in response to DNA damage ( 12,  13).	transcription
73234	1	336363	7	NULL	NULL	0	NULL	P/CAF	GP		does not acetylate					 GATA-1 	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20853_s_291	10779504	P/CAF does not acetylate GATA-1 ( 21), and the carboxyl-terminal acetylation site of p53 is preferentially acetylated by p300 compared with P/CAF ( 19).	transcription
73236	2	336363	7	NULL	NULL	NULL	NULL	p300	GP		acetylate		preferentially			p53	GP		carboxyl-terminal acetylation site		NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_275_27_20853_s_291	10779504	P/CAF does not acetylate GATA-1 ( 21), and the carboxyl-terminal acetylation site of p53 is preferentially acetylated by p300 compared with P/CAF ( 19).	transcription
73254	1	336364	7	NULL	NULL	0	NULL	small oligonucleotides	NucleicAcid		stabilize			p53 consensus site		p300.p53 complex	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_15_13431_s_263	12499368	Using purified p300 and p53 proteins, we show that small oligonucleotides containing the p53 consensus site (Fig.  9 A) or supercoiled plasmid DNA containing the p53 consensus site (Fig.  9 B), can promote a striking stabilization of the p300.p53 complex after the addition of acetyl-CoA (Fig.  9,  A and  B,  lane 12), relative to nonspecific DNA (Fig.  9,  A and  B,  lane 11 versus 12).	transcription
73255	2	336364	7	NULL	NULL	0	NULL	statement 1	Process		occur after					acetyl-CoA	Chemical	addition of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_15_13431_s_263	12499368	Using purified p300 and p53 proteins, we show that small oligonucleotides containing the p53 consensus site (Fig.  9 A) or supercoiled plasmid DNA containing the p53 consensus site (Fig.  9 B), can promote a striking stabilization of the p300.p53 complex after the addition of acetyl-CoA (Fig.  9,  A and  B,  lane 12), relative to nonspecific DNA (Fig.  9,  A and  B,  lane 11 versus 12).	transcription
73256	3	336364	7	NULL	NULL	0	NULL	supercoiled plasmid DNA	NucleicAcid		stabilize			p53 consensus site		p300.p53 complex	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_15_13431_s_263	12499368	Using purified p300 and p53 proteins, we show that small oligonucleotides containing the p53 consensus site (Fig.  9 A) or supercoiled plasmid DNA containing the p53 consensus site (Fig.  9 B), can promote a striking stabilization of the p300.p53 complex after the addition of acetyl-CoA (Fig.  9,  A and  B,  lane 12), relative to nonspecific DNA (Fig.  9,  A and  B,  lane 11 versus 12).	transcription
73258	4	336364	7	NULL	NULL	0	NULL	statement 3	Process		occur after					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_15_13431_s_263	12499368	Using purified p300 and p53 proteins, we show that small oligonucleotides containing the p53 consensus site (Fig.  9 A) or supercoiled plasmid DNA containing the p53 consensus site (Fig.  9 B), can promote a striking stabilization of the p300.p53 complex after the addition of acetyl-CoA (Fig.  9,  A and  B,  lane 12), relative to nonspecific DNA (Fig.  9,  A and  B,  lane 11 versus 12).	transcription
73259	1	336365	7	NULL	NULL	0	NULL	p53	GP		associate with					U6	GP			promoter	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_8_3247_s_179	15798209	Second, low levels of p53 associate with the U6 promoter prior to stress and UV light stimulates p53 promoter association, but this p53 is not acetylated to a significant degree.	transcription
73260	2	336365	7	NULL	NULL	0	NULL	statement 1	Process		occur prior to					stress	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_8_3247_s_179	15798209	Second, low levels of p53 associate with the U6 promoter prior to stress and UV light stimulates p53 promoter association, but this p53 is not acetylated to a significant degree.	transcription
73261	3	336365	7	NULL	NULL	0	NULL	UVlight	PhysicalPhenomenon		stimulate					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_8_3247_s_179	15798209	Second, low levels of p53 associate with the U6 promoter prior to stress and UV light stimulates p53 promoter association, but this p53 is not acetylated to a significant degree.	transcription
73262	4	336365	7	NULL	NULL	0	NULL	statement 3	Process		does not acetylate					p53	GP				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_8_3247_s_179	15798209	Second, low levels of p53 associate with the U6 promoter prior to stress and UV light stimulates p53 promoter association, but this p53 is not acetylated to a significant degree.	transcription
73264	1	336366	7	NULL	NULL	0	NULL	p300	GP		clamped to					p53	GP	acetylated			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_22_10083_s_311	15509808	Thus, the observation that acetylation of p53 enhances its transcriptional activity can be explained in part by the clamping of p300 to acetylated p53 when p53 is DNA bound ( ).	transcription
73265	2	336366	7	NULL	NULL	0	NULL	p53	GP		bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_22_10083_s_311	15509808	Thus, the observation that acetylation of p53 enhances its transcriptional activity can be explained in part by the clamping of p300 to acetylated p53 when p53 is DNA bound ( ).	transcription
73268	3	336366	7	NULL	NULL	0	NULL	p53	GP	acetylation of	enhance					p53	GP	transcriptional activity of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_24_22_10083_s_311	15509808	Thus, the observation that acetylation of p53 enhances its transcriptional activity can be explained in part by the clamping of p300 to acetylated p53 when p53 is DNA bound ( ).	transcription
73271	1	336367	7	NULL	NULL	0	NULL	p53	GP		bind					Daxx	GP	yeast			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_50566_s_204	15364927	We showed above that several p53 mutants that mimic acetylated or phosphorylated p53 abolished binding of p53 to Daxx in yeast ( Fig. 1 G).	transcription
73274	2	336367	7	NULL	NULL	0	NULL	p53	GP	mutant mimicking acetylated	abolish					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_50566_s_204	15364927	We showed above that several p53 mutants that mimic acetylated or phosphorylated p53 abolished binding of p53 to Daxx in yeast ( Fig. 1 G).	transcription
73276	3	336367	7	NULL	NULL	NULL	NULL	p53	GP	mutant mimicking phosphorylated	abolish					statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_48_50566_s_204	15364927	We showed above that several p53 mutants that mimic acetylated or phosphorylated p53 abolished binding of p53 to Daxx in yeast ( Fig. 1 G).	transcription
73277	1	336368	7	NULL	NULL	0	NULL	 p53	GP	acetylation of	is a type of					transient event	Process				NULL		0	NULL	NULL	NULL	gw60_embo_20_6_1331_s_69	11250899	As shown in Figure  1A, p53 acetylation is a transient event and, after an initial increase, the abundance of acetylated p53 decreased due to the activity of a putative p53 deacetylase.	transcription
73278	2	336368	7	NULL	NULL	0	NULL	p53	GP	acetylated	decrease					putative p53 deacetylase	GP	due to activity of			NULL		0	NULL	NULL	NULL	gw60_embo_20_6_1331_s_69	11250899	As shown in Figure  1A, p53 acetylation is a transient event and, after an initial increase, the abundance of acetylated p53 decreased due to the activity of a putative p53 deacetylase.	transcription
73280	3	336368	7	NULL	NULL	0	NULL	statement 2	Process		occur after					p53	GP	initial increase of acetylated			NULL		0	NULL	NULL	NULL	gw60_embo_20_6_1331_s_69	11250899	As shown in Figure  1A, p53 acetylation is a transient event and, after an initial increase, the abundance of acetylated p53 decreased due to the activity of a putative p53 deacetylase.	transcription
73282	1	336369	7	NULL	NULL	0	NULL	PCAF	GP		acetylates					p53	GP		lysine 320		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_19_20035_s_34	14769800	PCAF also acetylates p53 at lysine 320 in response to DNA damage signals and activates the activity of p53 ( ).	transcription
73283	2	336369	7	NULL	NULL	0	NULL	statement 1	Process		in response to					DNA damage signals	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_19_20035_s_34	14769800	PCAF also acetylates p53 at lysine 320 in response to DNA damage signals and activates the activity of p53 ( ).	transcription
73284	3	336369	7	NULL	NULL	0	NULL	statement 1	Process		activates 					p53	GP	activity of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_19_20035_s_34	14769800	PCAF also acetylates p53 at lysine 320 in response to DNA damage signals and activates the activity of p53 ( ).	transcription
73285	1	336370	7	NULL	NULL	0	NULL	PCAF	GP		acetylate		efficiently			p53	GP				NULL	in vitro	0	NULL	NULL	NULL	gw60_molcellbiol_19_2_1202_s_78	9891054	This result indicated that PCAF efficiently acetylates p53 in vitro and that PCAF and p300 target distinct residues within p53.	transcription
73286	2	336370	7	NULL	NULL	0	NULL	PCAF	GP		target					p53	GP		distinct residues		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_2_1202_s_78	9891054	This result indicated that PCAF efficiently acetylates p53 in vitro and that PCAF and p300 target distinct residues within p53.	transcription
73287	3	336370	7	NULL	NULL	0	NULL	p300	GP		target					p53	GP		distinct residues		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_2_1202_s_78	9891054	This result indicated that PCAF efficiently acetylates p53 in vitro and that PCAF and p300 target distinct residues within p53.	transcription
73288	1	336371	7	NULL	NULL	0	NULL	ZBP-89	GP		bind		directly			p21waf1	GP			promoter	NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_14_4670_s_378	11416144	ZBP-89 binds directly to the p21waf1 promoter ( 5,  19), but, in the absence of p53, ZBP-89 requires recruitment of a histone acetylase and inhibition of deacetylase activity ( 5).	transcription
73289	2	336371	7	NULL	NULL	0	NULL	statement 1	Process		in the absence of					p53	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_14_4670_s_378	11416144	ZBP-89 binds directly to the p21waf1 promoter ( 5,  19), but, in the absence of p53, ZBP-89 requires recruitment of a histone acetylase and inhibition of deacetylase activity ( 5).	transcription
73290	3	336371	7	NULL	NULL	NULL	NULL	 ZBP-89 	GP		requires					histone acetylase	GP	recruitment of			NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_14_4670_s_378	11416144	ZBP-89 binds directly to the p21waf1 promoter ( 5,  19), but, in the absence of p53, ZBP-89 requires recruitment of a histone acetylase and inhibition of deacetylase activity ( 5).	transcription
73291	4	336371	7	NULL	NULL	0	NULL	ZBP-89			requires					deacetylase activity	Process	inhibition of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_14_4670_s_378	11416144	ZBP-89 binds directly to the p21waf1 promoter ( 5,  19), but, in the absence of p53, ZBP-89 requires recruitment of a histone acetylase and inhibition of deacetylase activity ( 5).	transcription
73292	1	336372	7	NULL	NULL	0	NULL	CBP	GP		acetylate					p53	GP				NULL		0	NULL	NULL	NULL	gw60_molcell_3_1_125_s_24	10024886	For example, CBP can acetylate the tumor suppressor protein p53, and this modification stimulates its DNA binding activity ( Gu and Roeder 1997  ).	transcription
73293	2	336372	7	NULL	NULL	0	NULL	p53	GP		bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_molcell_3_1_125_s_24	10024886	For example, CBP can acetylate the tumor suppressor protein p53, and this modification stimulates its DNA binding activity ( Gu and Roeder 1997  ).	transcription
73294	3	336372	7	NULL	NULL	0	NULL	statement 1	Process		stimulate					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_3_1_125_s_24	10024886	For example, CBP can acetylate the tumor suppressor protein p53, and this modification stimulates its DNA binding activity ( Gu and Roeder 1997  ).	transcription
73295	4	336372	7	NULL	NULL	0	NULL	p53	GP		is a type of					tumor suppressor protein	GP				NULL		0	NULL	NULL	NULL	gw60_molcell_3_1_125_s_24	10024886	For example, CBP can acetylate the tumor suppressor protein p53, and this modification stimulates its DNA binding activity ( Gu and Roeder 1997  ).	transcription
73297	1	336373	7	NULL	NULL	0	NULL	p300	GP		acetylate					p53	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_95_22_12924_s_136	9789016	For example, in addition to histones, p300 will acetylate the tumor suppressor protein, p53, thereby enhancing its DNA-binding activity  in vitro ( 37).	transcription
73298	2	336373	7	NULL	NULL	0	NULL	p300	GP		acetylate					histones	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_95_22_12924_s_136	9789016	For example, in addition to histones, p300 will acetylate the tumor suppressor protein, p53, thereby enhancing its DNA-binding activity  in vitro ( 37).	transcription
73299	3	336373	7	NULL	NULL	NULL	NULL	p53	GP		bind					DNA	NucleicAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_pnas_95_22_12924_s_136	9789016	For example, in addition to histones, p300 will acetylate the tumor suppressor protein, p53, thereby enhancing its DNA-binding activity  in vitro ( 37).	transcription
73300	4	336373	7	NULL	NULL	0	NULL	p53	GP		is a type of					tumor suppressor protein	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_95_22_12924_s_136	9789016	For example, in addition to histones, p300 will acetylate the tumor suppressor protein, p53, thereby enhancing its DNA-binding activity  in vitro ( 37).	transcription
73301	1	336374	7	NULL	NULL	0	NULL	HDIs	GP		is a type of					transcriptional activator	GP				NULL		0	NULL	NULL	NULL	gw70_febslett_570_1_37_s_5	15251435	Hypotheses have been generated which suggest that HDIs are transcriptional activators  that disrupt the balance between histone deacetylase (HDAC) and histone acetyl transferase  (HAT) activity resulting in hyperacetylation of nucleosomal histones and non-histone  proteins, such as the transcription factor p53 [  5 and   6].	transcription
73302	2	336374	7	NULL	NULL	0	NULL	HDAC	GP	activity of	is in balance with					HAT	GP	activity of			NULL		0	NULL	NULL	NULL	gw70_febslett_570_1_37_s_5	15251435	Hypotheses have been generated which suggest that HDIs are transcriptional activators  that disrupt the balance between histone deacetylase (HDAC) and histone acetyl transferase  (HAT) activity resulting in hyperacetylation of nucleosomal histones and non-histone  proteins, such as the transcription factor p53 [  5 and   6].	transcription
73303	3	336374	7	NULL	NULL	0	NULL	HDI	GP		disrupt					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_febslett_570_1_37_s_5	15251435	Hypotheses have been generated which suggest that HDIs are transcriptional activators  that disrupt the balance between histone deacetylase (HDAC) and histone acetyl transferase  (HAT) activity resulting in hyperacetylation of nucleosomal histones and non-histone  proteins, such as the transcription factor p53 [  5 and   6].	transcription
73304	4	336374	7	NULL	NULL	0	NULL	statement 3	Process		result in					nucleosomal histones	GP	hyperacetylation of			NULL		0	NULL	NULL	NULL	gw70_febslett_570_1_37_s_5	15251435	Hypotheses have been generated which suggest that HDIs are transcriptional activators  that disrupt the balance between histone deacetylase (HDAC) and histone acetyl transferase  (HAT) activity resulting in hyperacetylation of nucleosomal histones and non-histone  proteins, such as the transcription factor p53 [  5 and   6].	transcription
73305	5	336374	7	NULL	NULL	0	NULL	statement 3	Process		result in					p53	GP	hyperacetylation of			NULL		0	NULL	NULL	NULL	gw70_febslett_570_1_37_s_5	15251435	Hypotheses have been generated which suggest that HDIs are transcriptional activators  that disrupt the balance between histone deacetylase (HDAC) and histone acetyl transferase  (HAT) activity resulting in hyperacetylation of nucleosomal histones and non-histone  proteins, such as the transcription factor p53 [  5 and   6].	transcription
73306	6	336374	7	NULL	NULL	0	NULL	p53	GP		is a type of					transcription factor	GP				NULL		0	NULL	NULL	NULL	gw70_febslett_570_1_37_s_5	15251435	Hypotheses have been generated which suggest that HDIs are transcriptional activators  that disrupt the balance between histone deacetylase (HDAC) and histone acetyl transferase  (HAT) activity resulting in hyperacetylation of nucleosomal histones and non-histone  proteins, such as the transcription factor p53 [  5 and   6].	transcription
73307	7	336374	7	NULL	NULL	0	NULL	p53	GP		is a type of					non-histone proteins	GP				NULL		0	NULL	NULL	NULL	gw70_febslett_570_1_37_s_5	15251435	Hypotheses have been generated which suggest that HDIs are transcriptional activators  that disrupt the balance between histone deacetylase (HDAC) and histone acetyl transferase  (HAT) activity resulting in hyperacetylation of nucleosomal histones and non-histone  proteins, such as the transcription factor p53 [  5 and   6].	transcription
73308	8	336374	7	NULL	NULL	0	NULL	HDAC	GP		is					histone deacetylase	GP				NULL		0	NULL	NULL	NULL	gw70_febslett_570_1_37_s_5	15251435	Hypotheses have been generated which suggest that HDIs are transcriptional activators  that disrupt the balance between histone deacetylase (HDAC) and histone acetyl transferase  (HAT) activity resulting in hyperacetylation of nucleosomal histones and non-histone  proteins, such as the transcription factor p53 [  5 and   6].	transcription
73309	9	336374	7	NULL	NULL	0	NULL	HAT	GP		is					histone acetyl transferase	GP				NULL		0	NULL	NULL	NULL	gw70_febslett_570_1_37_s_5	15251435	Hypotheses have been generated which suggest that HDIs are transcriptional activators  that disrupt the balance between histone deacetylase (HDAC) and histone acetyl transferase  (HAT) activity resulting in hyperacetylation of nucleosomal histones and non-histone  proteins, such as the transcription factor p53 [  5 and   6].	transcription
73310	1	336375	7	NULL	NULL	0	NULL	Myc oncogene	GP		induce					p53	GP	phosphorylation of			NULL		0	NULL	NULL	NULL	gw70_nature_434_7035_864_s_106	15829956	Furthermore, unlike phosphorylations of p53 and H2AX induced  by the Myc oncogene, which are a consequence of oxygen radical generation 11, the DNA damage response in our experiments was only marginally repressed by the  antioxidant  N-acetyl- l-cysteine (NAC;  Fig. 4a and  Supplementary Figs S4d, S5b, c).	transcription
73311	2	336375	7	NULL	NULL	NULL	NULL	Myc oncogene	GP		induce					H2AX	GP	phosphorylation of			NULL		NULL	NULL	NULL	NULL	gw70_nature_434_7035_864_s_106	15829956	Furthermore, unlike phosphorylations of p53 and H2AX induced  by the Myc oncogene, which are a consequence of oxygen radical generation 11, the DNA damage response in our experiments was only marginally repressed by the  antioxidant  N-acetyl- l-cysteine (NAC;  Fig. 4a and  Supplementary Figs S4d, S5b, c).	transcription
73312	3	336375	7	NULL	NULL	0	NULL	statement 1	Process		as a consequence of					oxygen radical generation	Process				NULL		0	NULL	NULL	NULL	gw70_nature_434_7035_864_s_106	15829956	Furthermore, unlike phosphorylations of p53 and H2AX induced  by the Myc oncogene, which are a consequence of oxygen radical generation 11, the DNA damage response in our experiments was only marginally repressed by the  antioxidant  N-acetyl- l-cysteine (NAC;  Fig. 4a and  Supplementary Figs S4d, S5b, c).	transcription
73313	4	336375	7	NULL	NULL	0	NULL	statement 2	Process		as a consequence of					oxygen radical generation	Process				NULL		0	NULL	NULL	NULL	gw70_nature_434_7035_864_s_106	15829956	Furthermore, unlike phosphorylations of p53 and H2AX induced  by the Myc oncogene, which are a consequence of oxygen radical generation 11, the DNA damage response in our experiments was only marginally repressed by the  antioxidant  N-acetyl- l-cysteine (NAC;  Fig. 4a and  Supplementary Figs S4d, S5b, c).	transcription
73314	5	336375	7	NULL	NULL	0	NULL	NAC	Chemical		repress		marginally			DNA damage response	Process				NULL		0	NULL	NULL	NULL	gw70_nature_434_7035_864_s_106	15829956	Furthermore, unlike phosphorylations of p53 and H2AX induced  by the Myc oncogene, which are a consequence of oxygen radical generation 11, the DNA damage response in our experiments was only marginally repressed by the  antioxidant  N-acetyl- l-cysteine (NAC;  Fig. 4a and  Supplementary Figs S4d, S5b, c).	transcription
73315	6	336375	7	NULL	NULL	0	NULL	NAC	Chemical		is					N-acetyl- l-cysteine	Chemical				NULL		0	NULL	NULL	NULL	gw70_nature_434_7035_864_s_106	15829956	Furthermore, unlike phosphorylations of p53 and H2AX induced  by the Myc oncogene, which are a consequence of oxygen radical generation 11, the DNA damage response in our experiments was only marginally repressed by the  antioxidant  N-acetyl- l-cysteine (NAC;  Fig. 4a and  Supplementary Figs S4d, S5b, c).	transcription
73316	7	336375	7	NULL	NULL	0	NULL	NAC	Chemical		is a type of					antioxidant	Chemical				NULL		0	NULL	NULL	NULL	gw70_nature_434_7035_864_s_106	15829956	Furthermore, unlike phosphorylations of p53 and H2AX induced  by the Myc oncogene, which are a consequence of oxygen radical generation 11, the DNA damage response in our experiments was only marginally repressed by the  antioxidant  N-acetyl- l-cysteine (NAC;  Fig. 4a and  Supplementary Figs S4d, S5b, c).	transcription
73317	1	336376	7	NULL	NULL	0	NULL	acetyl-CoA	Chemical		promote					p53	GP	acetylation of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_174	14612423	Using the p300 acetylation reaction where acetyl-CoA promotes p53 acetylation in a sequence-specific DNA-dependent manner (Fig.  3B, lane 2 versus lane 1), the PXXP repeat peptide was found to be a specific inhibitor of DNA-dependent acetylation (Fig.  3B, lanes 8 to 10 versus lanes 2 to 6).	transcription
73318	2	336376	7	NULL	NULL	0	NULL	statement 1	Process		depends on					DNA	NucleicAcid	sequence-specific			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_174	14612423	Using the p300 acetylation reaction where acetyl-CoA promotes p53 acetylation in a sequence-specific DNA-dependent manner (Fig.  3B, lane 2 versus lane 1), the PXXP repeat peptide was found to be a specific inhibitor of DNA-dependent acetylation (Fig.  3B, lanes 8 to 10 versus lanes 2 to 6).	transcription
73319	3	336376	7	NULL	NULL	0	NULL	acetylation	Process		depends on					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_174	14612423	Using the p300 acetylation reaction where acetyl-CoA promotes p53 acetylation in a sequence-specific DNA-dependent manner (Fig.  3B, lane 2 versus lane 1), the PXXP repeat peptide was found to be a specific inhibitor of DNA-dependent acetylation (Fig.  3B, lanes 8 to 10 versus lanes 2 to 6).	transcription
73320	4	336376	7	NULL	NULL	0	NULL	PXXP repeat peptide	AminoAcid		inhibitor of		specific			statement 3	GP				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_23_23_8846_s_174	14612423	Using the p300 acetylation reaction where acetyl-CoA promotes p53 acetylation in a sequence-specific DNA-dependent manner (Fig.  3B, lane 2 versus lane 1), the PXXP repeat peptide was found to be a specific inhibitor of DNA-dependent acetylation (Fig.  3B, lanes 8 to 10 versus lanes 2 to 6).	transcription
73321	1	336377	7	NULL	NULL	0	NULL	p53	GP		induce					ROS	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_17_17765_s_92	14764594	To examine whether ROS induction by p53 is critical for senescence and Bcl-xL and E1B-19K inhibit p53-induced senescence by preventing ROS generation, we examined the effects of anti-oxidants,  N-acetyl-L-cysteine (NAC) and 1-pyrrolydine dithiocarbamate (PDTC).	transcription
73322	2	336377	7	NULL	NULL	0	NULL	statement 1	Process		critical for					senescence	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_17_17765_s_92	14764594	To examine whether ROS induction by p53 is critical for senescence and Bcl-xL and E1B-19K inhibit p53-induced senescence by preventing ROS generation, we examined the effects of anti-oxidants,  N-acetyl-L-cysteine (NAC) and 1-pyrrolydine dithiocarbamate (PDTC).	transcription
73323	3	336377	7	NULL	NULL	0	NULL	Bcl-xL	GP		inhibit					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_17_17765_s_92	14764594	To examine whether ROS induction by p53 is critical for senescence and Bcl-xL and E1B-19K inhibit p53-induced senescence by preventing ROS generation, we examined the effects of anti-oxidants,  N-acetyl-L-cysteine (NAC) and 1-pyrrolydine dithiocarbamate (PDTC).	transcription
73324	4	336377	7	NULL	NULL	0	NULL	E1B-19K	GP		inhibit					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_17_17765_s_92	14764594	To examine whether ROS induction by p53 is critical for senescence and Bcl-xL and E1B-19K inhibit p53-induced senescence by preventing ROS generation, we examined the effects of anti-oxidants,  N-acetyl-L-cysteine (NAC) and 1-pyrrolydine dithiocarbamate (PDTC).	transcription
73325	5	336377	7	NULL	NULL	0	NULL	statement 3	Process		occur by					ROS	Chemical	preventing generation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_17_17765_s_92	14764594	To examine whether ROS induction by p53 is critical for senescence and Bcl-xL and E1B-19K inhibit p53-induced senescence by preventing ROS generation, we examined the effects of anti-oxidants,  N-acetyl-L-cysteine (NAC) and 1-pyrrolydine dithiocarbamate (PDTC).	transcription
73326	6	336377	7	NULL	NULL	0	NULL	statement 4	Process		occur by					ROS	Chemical	preventing generation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_17_17765_s_92	14764594	To examine whether ROS induction by p53 is critical for senescence and Bcl-xL and E1B-19K inhibit p53-induced senescence by preventing ROS generation, we examined the effects of anti-oxidants,  N-acetyl-L-cysteine (NAC) and 1-pyrrolydine dithiocarbamate (PDTC).	transcription
73327	7	336377	7	NULL	NULL	0	NULL	NAC	Chemical		is					N-acetyl-L-cysteine	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_17_17765_s_92	14764594	To examine whether ROS induction by p53 is critical for senescence and Bcl-xL and E1B-19K inhibit p53-induced senescence by preventing ROS generation, we examined the effects of anti-oxidants,  N-acetyl-L-cysteine (NAC) and 1-pyrrolydine dithiocarbamate (PDTC).	transcription
73328	8	336377	7	NULL	NULL	0	NULL	PDTC	Chemical		is					1-pyrrolydine dithiocarbamate	Chemical				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_17_17765_s_92	14764594	To examine whether ROS induction by p53 is critical for senescence and Bcl-xL and E1B-19K inhibit p53-induced senescence by preventing ROS generation, we examined the effects of anti-oxidants,  N-acetyl-L-cysteine (NAC) and 1-pyrrolydine dithiocarbamate (PDTC).	transcription
73329	1	336378	7	NULL	NULL	NULL	NULL	E1A protein	GP	human adenovirus	bind					retinoblastoma tumor suppressor family 	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_23_3104_s_18	11731475	In the case of human adenoviruses, binding of the viral early region 1A (E1A) protein with either the retinoblastoma tumor suppressor family or p300/CBP/p400 histone acetyl transferases induces the activation, stabilization, and accumulation of p53 (Chiou and White 1997  ; Querido et al. 1997b  ; Samuelson and Lowe 1997  ).	transcription
73330	2	336378	7	NULL	NULL	NULL	NULL	E1A protein	GP	human adenovirus	bind					p300/CBP/p400 histone acetyl transferases 	GP				NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_23_3104_s_18	11731475	In the case of human adenoviruses, binding of the viral early region 1A (E1A) protein with either the retinoblastoma tumor suppressor family or p300/CBP/p400 histone acetyl transferases induces the activation, stabilization, and accumulation of p53 (Chiou and White 1997  ; Querido et al. 1997b  ; Samuelson and Lowe 1997  ).	transcription
73331	3	336378	7	NULL	NULL	0	NULL	statement 1	Process		induce					p53	GP	activation of			NULL		0	NULL	NULL	NULL	gw60_genesdev_15_23_3104_s_18	11731475	In the case of human adenoviruses, binding of the viral early region 1A (E1A) protein with either the retinoblastoma tumor suppressor family or p300/CBP/p400 histone acetyl transferases induces the activation, stabilization, and accumulation of p53 (Chiou and White 1997  ; Querido et al. 1997b  ; Samuelson and Lowe 1997  ).	transcription
73332	4	336378	7	NULL	NULL	0	NULL	statement 1	Process		induce					p53	GP	stabilization of			NULL		0	NULL	NULL	NULL	gw60_genesdev_15_23_3104_s_18	11731475	In the case of human adenoviruses, binding of the viral early region 1A (E1A) protein with either the retinoblastoma tumor suppressor family or p300/CBP/p400 histone acetyl transferases induces the activation, stabilization, and accumulation of p53 (Chiou and White 1997  ; Querido et al. 1997b  ; Samuelson and Lowe 1997  ).	transcription
73333	5	336378	7	NULL	NULL	0	NULL	statement 1	Process		induce					p53	GP	accumulation of			NULL		0	NULL	NULL	NULL	gw60_genesdev_15_23_3104_s_18	11731475	In the case of human adenoviruses, binding of the viral early region 1A (E1A) protein with either the retinoblastoma tumor suppressor family or p300/CBP/p400 histone acetyl transferases induces the activation, stabilization, and accumulation of p53 (Chiou and White 1997  ; Querido et al. 1997b  ; Samuelson and Lowe 1997  ).	transcription
73334	6	336378	7	NULL	NULL	NULL	NULL	statement 2	Process		induce					p53	GP	activation of			NULL		NULL	NULL	NULL	NULL	gw60_genesdev_15_23_3104_s_18	11731475	In the case of human adenoviruses, binding of the viral early region 1A (E1A) protein with either the retinoblastoma tumor suppressor family or p300/CBP/p400 histone acetyl transferases induces the activation, stabilization, and accumulation of p53 (Chiou and White 1997  ; Querido et al. 1997b  ; Samuelson and Lowe 1997  ).	transcription
73335	7	336378	7	NULL	NULL	0	NULL	statement 2	Process		induce					p53	GP	stabilization of			NULL		0	NULL	NULL	NULL	gw60_genesdev_15_23_3104_s_18	11731475	In the case of human adenoviruses, binding of the viral early region 1A (E1A) protein with either the retinoblastoma tumor suppressor family or p300/CBP/p400 histone acetyl transferases induces the activation, stabilization, and accumulation of p53 (Chiou and White 1997  ; Querido et al. 1997b  ; Samuelson and Lowe 1997  ).	transcription
73336	8	336378	7	NULL	NULL	0	NULL	statement 2	Process		induce					p53	GP	accumulation of			NULL		0	NULL	NULL	NULL	gw60_genesdev_15_23_3104_s_18	11731475	In the case of human adenoviruses, binding of the viral early region 1A (E1A) protein with either the retinoblastoma tumor suppressor family or p300/CBP/p400 histone acetyl transferases induces the activation, stabilization, and accumulation of p53 (Chiou and White 1997  ; Querido et al. 1997b  ; Samuelson and Lowe 1997  ).	transcription
73337	9	336378	7	NULL	NULL	0	NULL	E1A protein	GP		is					viral early region 1A protein	GP				NULL		0	NULL	NULL	NULL	gw60_genesdev_15_23_3104_s_18	11731475	In the case of human adenoviruses, binding of the viral early region 1A (E1A) protein with either the retinoblastoma tumor suppressor family or p300/CBP/p400 histone acetyl transferases induces the activation, stabilization, and accumulation of p53 (Chiou and White 1997  ; Querido et al. 1997b  ; Samuelson and Lowe 1997  ).	transcription
73338	10	336378	7	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_genesdev_15_23_3104_s_18	11731475	In the case of human adenoviruses, binding of the viral early region 1A (E1A) protein with either the retinoblastoma tumor suppressor family or p300/CBP/p400 histone acetyl transferases induces the activation, stabilization, and accumulation of p53 (Chiou and White 1997  ; Querido et al. 1997b  ; Samuelson and Lowe 1997  ).	transcription
73339	1	336379	7	NULL	NULL	0	NULL	CBP/p300	GP		acetylates					p53	GP				NULL		0	NULL	NULL	NULL	gw60_molcell_8_1_57_s_19	11511360	Acetylation of p53 by the histone acetyl transferases CBP/p300 and PCAF activates DNA binding in vitro and each HAT can coactivate p53-dependent transcription in transient expression experiments      (Gu and Roeder, 1997  ; Avantaggiati et al., 1997  ; Lill et al., 1997  ; Scolnick et al., 1997  ; Liu et al., 1999  ).	transcription
73340	2	336379	7	NULL	NULL	0	NULL	PCAF	GP		acetylates					p53	GP				NULL		0	NULL	NULL	NULL	gw60_molcell_8_1_57_s_19	11511360	Acetylation of p53 by the histone acetyl transferases CBP/p300 and PCAF activates DNA binding in vitro and each HAT can coactivate p53-dependent transcription in transient expression experiments      (Gu and Roeder, 1997  ; Avantaggiati et al., 1997  ; Lill et al., 1997  ; Scolnick et al., 1997  ; Liu et al., 1999  ).	transcription
73341	4	336379	7	NULL	NULL	NULL	NULL	statement 1	Process		activates					statement 3	Process				NULL		NULL	NULL	NULL	NULL	gw60_molcell_8_1_57_s_19	11511360	Acetylation of p53 by the histone acetyl transferases CBP/p300 and PCAF activates DNA binding in vitro and each HAT can coactivate p53-dependent transcription in transient expression experiments      (Gu and Roeder, 1997  ; Avantaggiati et al., 1997  ; Lill et al., 1997  ; Scolnick et al., 1997  ; Liu et al., 1999  ).	transcription
73342	3	336379	7	NULL	NULL	NULL	NULL	p53	GP		bind					DNA	NucleicAcid				NULL	in vitro	NULL	NULL	NULL	NULL	gw60_molcell_8_1_57_s_19	11511360	Acetylation of p53 by the histone acetyl transferases CBP/p300 and PCAF activates DNA binding in vitro and each HAT can coactivate p53-dependent transcription in transient expression experiments      (Gu and Roeder, 1997  ; Avantaggiati et al., 1997  ; Lill et al., 1997  ; Scolnick et al., 1997  ; Liu et al., 1999  ).	transcription
73343	5	336379	7	NULL	NULL	0	NULL	statement 2	Process		activates					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_8_1_57_s_19	11511360	Acetylation of p53 by the histone acetyl transferases CBP/p300 and PCAF activates DNA binding in vitro and each HAT can coactivate p53-dependent transcription in transient expression experiments      (Gu and Roeder, 1997  ; Avantaggiati et al., 1997  ; Lill et al., 1997  ; Scolnick et al., 1997  ; Liu et al., 1999  ).	transcription
73344	6	336379	7	NULL	NULL	0	NULL	transcription	Process		depends on					p53	GP				NULL		0	NULL	NULL	NULL	gw60_molcell_8_1_57_s_19	11511360	Acetylation of p53 by the histone acetyl transferases CBP/p300 and PCAF activates DNA binding in vitro and each HAT can coactivate p53-dependent transcription in transient expression experiments      (Gu and Roeder, 1997  ; Avantaggiati et al., 1997  ; Lill et al., 1997  ; Scolnick et al., 1997  ; Liu et al., 1999  ).	transcription
73345	7	336379	7	NULL	NULL	0	NULL	HAT	GP		coactivate					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_8_1_57_s_19	11511360	Acetylation of p53 by the histone acetyl transferases CBP/p300 and PCAF activates DNA binding in vitro and each HAT can coactivate p53-dependent transcription in transient expression experiments      (Gu and Roeder, 1997  ; Avantaggiati et al., 1997  ; Lill et al., 1997  ; Scolnick et al., 1997  ; Liu et al., 1999  ).	transcription
73346	8	336379	7	NULL	NULL	0	NULL	CBP/p300	GP		is a type of					histone acetyl transferases	GP				NULL		0	NULL	NULL	NULL	gw60_molcell_8_1_57_s_19	11511360	Acetylation of p53 by the histone acetyl transferases CBP/p300 and PCAF activates DNA binding in vitro and each HAT can coactivate p53-dependent transcription in transient expression experiments      (Gu and Roeder, 1997  ; Avantaggiati et al., 1997  ; Lill et al., 1997  ; Scolnick et al., 1997  ; Liu et al., 1999  ).	transcription
73347	9	336379	7	NULL	NULL	0	NULL	PCAF	GP		is a type of					histone acetyl transferases	GP				NULL		0	NULL	NULL	NULL	gw60_molcell_8_1_57_s_19	11511360	Acetylation of p53 by the histone acetyl transferases CBP/p300 and PCAF activates DNA binding in vitro and each HAT can coactivate p53-dependent transcription in transient expression experiments      (Gu and Roeder, 1997  ; Avantaggiati et al., 1997  ; Lill et al., 1997  ; Scolnick et al., 1997  ; Liu et al., 1999  ).	transcription
73348	1	336380	7	NULL	NULL	NULL	NULL	staurosporine	Chemical		result in		effectively			apoptosis	Process				NULL	SH-SY5Y cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_18128_s_126	10364268	Indeed, treatment of SH-SY5Y cells with staurosporine,  N-acetyl-D- erythro-sphingosine, or menadione effectively resulted in apoptosis as demonstrated by DNA ladder assay (Fig.  2 A), and yet none of these paradigms induced nuclear accumulation of p53 under identical conditions (Fig.  2 B), confirming that their apoptotic effects are likely to involve p53-independent mechanisms.	transcription
73349	2	336380	7	NULL	NULL	0	NULL	N-acetyl-D- erythro-sphingosine	Chemical		result in		effectively			apoptosis	Process				NULL	SH-SY5Y cells	0	NULL	NULL	NULL	gw60_jbiolchem_274_25_18128_s_126	10364268	Indeed, treatment of SH-SY5Y cells with staurosporine,  N-acetyl-D- erythro-sphingosine, or menadione effectively resulted in apoptosis as demonstrated by DNA ladder assay (Fig.  2 A), and yet none of these paradigms induced nuclear accumulation of p53 under identical conditions (Fig.  2 B), confirming that their apoptotic effects are likely to involve p53-independent mechanisms.	transcription
73350	3	336380	7	NULL	NULL	NULL	NULL	menadione	Chemical		result in		effectively			apoptosis	Process				NULL	SH-SY5Y cells	NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_18128_s_126	10364268	Indeed, treatment of SH-SY5Y cells with staurosporine,  N-acetyl-D- erythro-sphingosine, or menadione effectively resulted in apoptosis as demonstrated by DNA ladder assay (Fig.  2 A), and yet none of these paradigms induced nuclear accumulation of p53 under identical conditions (Fig.  2 B), confirming that their apoptotic effects are likely to involve p53-independent mechanisms.	transcription
73351	7	336380	7	NULL	NULL	NULL	NULL	apoptotic effects	Process		involve					p53-independent mechanism	Process				NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_18128_s_126	10364268	Indeed, treatment of SH-SY5Y cells with staurosporine,  N-acetyl-D- erythro-sphingosine, or menadione effectively resulted in apoptosis as demonstrated by DNA ladder assay (Fig.  2 A), and yet none of these paradigms induced nuclear accumulation of p53 under identical conditions (Fig.  2 B), confirming that their apoptotic effects are likely to involve p53-independent mechanisms.	transcription
73352	4	336380	7	NULL	NULL	NULL	NULL	statement 1	Process		does not involve					p53	GP	nuclear accumulation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_18128_s_126	10364268	Indeed, treatment of SH-SY5Y cells with staurosporine,  N-acetyl-D- erythro-sphingosine, or menadione effectively resulted in apoptosis as demonstrated by DNA ladder assay (Fig.  2 A), and yet none of these paradigms induced nuclear accumulation of p53 under identical conditions (Fig.  2 B), confirming that their apoptotic effects are likely to involve p53-independent mechanisms.	transcription
73353	5	336380	7	NULL	NULL	NULL	NULL	statement 2	Process		does not involve					p53	GP	nuclear accumulation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_18128_s_126	10364268	Indeed, treatment of SH-SY5Y cells with staurosporine,  N-acetyl-D- erythro-sphingosine, or menadione effectively resulted in apoptosis as demonstrated by DNA ladder assay (Fig.  2 A), and yet none of these paradigms induced nuclear accumulation of p53 under identical conditions (Fig.  2 B), confirming that their apoptotic effects are likely to involve p53-independent mechanisms.	transcription
73354	6	336380	7	NULL	NULL	NULL	NULL	statement 3	Process		does not involve					p53	GP	nuclear accumulation of			NULL		NULL	NULL	NULL	NULL	gw60_jbiolchem_274_25_18128_s_126	10364268	Indeed, treatment of SH-SY5Y cells with staurosporine,  N-acetyl-D- erythro-sphingosine, or menadione effectively resulted in apoptosis as demonstrated by DNA ladder assay (Fig.  2 A), and yet none of these paradigms induced nuclear accumulation of p53 under identical conditions (Fig.  2 B), confirming that their apoptotic effects are likely to involve p53-independent mechanisms.	transcription
73355	8	336380	7	NULL	NULL	0	NULL	statement 4	Process		confirms					statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_25_18128_s_126	10364268	Indeed, treatment of SH-SY5Y cells with staurosporine,  N-acetyl-D- erythro-sphingosine, or menadione effectively resulted in apoptosis as demonstrated by DNA ladder assay (Fig.  2 A), and yet none of these paradigms induced nuclear accumulation of p53 under identical conditions (Fig.  2 B), confirming that their apoptotic effects are likely to involve p53-independent mechanisms.	transcription
73356	9	336380	7	NULL	NULL	0	NULL	statement 5	Process		confirms					statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_25_18128_s_126	10364268	Indeed, treatment of SH-SY5Y cells with staurosporine,  N-acetyl-D- erythro-sphingosine, or menadione effectively resulted in apoptosis as demonstrated by DNA ladder assay (Fig.  2 A), and yet none of these paradigms induced nuclear accumulation of p53 under identical conditions (Fig.  2 B), confirming that their apoptotic effects are likely to involve p53-independent mechanisms.	transcription
73357	10	336380	7	NULL	NULL	0	NULL	statement 6	Process		confirms					statement 7	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_25_18128_s_126	10364268	Indeed, treatment of SH-SY5Y cells with staurosporine,  N-acetyl-D- erythro-sphingosine, or menadione effectively resulted in apoptosis as demonstrated by DNA ladder assay (Fig.  2 A), and yet none of these paradigms induced nuclear accumulation of p53 under identical conditions (Fig.  2 B), confirming that their apoptotic effects are likely to involve p53-independent mechanisms.	transcription
73358	1	336381	7	NULL	NULL	0	NULL	PID	GP		interacts with		specifically			p53	GP				NULL	in vitro	0	NULL	NULL	NULL	gw60_nature_408_6810_377_s_13	11099047	PID specifically interacts with p53 both  in vitro and  in vivo, and its expression reduces significantly the steady-state levels of acetylated p53.	transcription
73359	2	336381	7	NULL	NULL	NULL	NULL	PID	GP		interacts with		specifically			p53	GP				NULL	in vivo	NULL	NULL	NULL	NULL	gw60_nature_408_6810_377_s_13	11099047	PID specifically interacts with p53 both  in vitro and  in vivo, and its expression reduces significantly the steady-state levels of acetylated p53.	transcription
73360	3	336381	7	NULL	NULL	0	NULL	statement 1	Process	expression of	reduces		significantly			p53	GP	acetylated			NULL		0	NULL	NULL	NULL	gw60_nature_408_6810_377_s_13	11099047	PID specifically interacts with p53 both  in vitro and  in vivo, and its expression reduces significantly the steady-state levels of acetylated p53.	transcription
73361	4	336381	7	NULL	NULL	0	NULL	statement 2	Process	expression of	reduces		significantly			p53	GP	acetylated			NULL		0	NULL	NULL	NULL	gw60_nature_408_6810_377_s_13	11099047	PID specifically interacts with p53 both  in vitro and  in vivo, and its expression reduces significantly the steady-state levels of acetylated p53.	transcription
73362	1	336382	7	NULL	NULL	0	NULL	p300	GP		acetylate					p53	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23027_s_231	10438470	Recently, Gu and Roeder ( 59) reported that p53 is acetylated by p300, a known histone acetyltransferase and transcriptional coactivator that is physically associated with p53.	transcription
73363	2	336382	7	NULL	NULL	0	NULL	p300	GP		associate with		physically			p53	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23027_s_231	10438470	Recently, Gu and Roeder ( 59) reported that p53 is acetylated by p300, a known histone acetyltransferase and transcriptional coactivator that is physically associated with p53.	transcription
73364	3	336382	7	NULL	NULL	0	NULL	p300	GP		is a type of					histone acetyltransferase	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23027_s_231	10438470	Recently, Gu and Roeder ( 59) reported that p53 is acetylated by p300, a known histone acetyltransferase and transcriptional coactivator that is physically associated with p53.	transcription
73365	4	336382	7	NULL	NULL	0	NULL	p300	GP		is a type of					transcriptional coactivator	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_33_23027_s_231	10438470	Recently, Gu and Roeder ( 59) reported that p53 is acetylated by p300, a known histone acetyltransferase and transcriptional coactivator that is physically associated with p53.	transcription
73366	1	336383	7	NULL	NULL	0	NULL	p53	GP		interacts with					p300	GP				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_276_42_11495913_s_5	11495913	Furthermore, interaction  of p53 with the transcriptional coactivator p300 was induced, and Lys(382)  of p53 was acetylated.	transcription
73367	2	336383	7	NULL	NULL	0	NULL	statement 1	Process		acetylate					p53	GP		Lys(382)		NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_276_42_11495913_s_5	11495913	Furthermore, interaction  of p53 with the transcriptional coactivator p300 was induced, and Lys(382)  of p53 was acetylated.	transcription
73368	3	336383	7	NULL	NULL	0	NULL	p300	GP		is a type of					transcriptional coactivator	GP				NULL		0	NULL	NULL	NULL	abs-batch0650-0679_j-biol-chem_276_42_11495913_s_5	11495913	Furthermore, interaction  of p53 with the transcriptional coactivator p300 was induced, and Lys(382)  of p53 was acetylated.	transcription
73369	1	336384	7	NULL	NULL	0	NULL	p53	GP	site-specific;;acetylation of	depends on					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_7_2782_s_29	16537920	Dornan et al. reported that site-specific acetylation of p53 was DNA dependent; deletion of the p53 proline repeat allows p53 to bind to  p21, but p53 was unable to be acetylated, indicating that proline-directed acetylation of p53 is a post-DNA binding event ( ,  ).	transcription
73370	2	336384	7	NULL	NULL	0	NULL	p53	GP		bind					p21	GP				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_7_2782_s_29	16537920	Dornan et al. reported that site-specific acetylation of p53 was DNA dependent; deletion of the p53 proline repeat allows p53 to bind to  p21, but p53 was unable to be acetylated, indicating that proline-directed acetylation of p53 is a post-DNA binding event ( ,  ).	transcription
73371	3	336384	7	NULL	NULL	0	NULL	p53	GP	deletion of	allows			proline repeat		statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_7_2782_s_29	16537920	Dornan et al. reported that site-specific acetylation of p53 was DNA dependent; deletion of the p53 proline repeat allows p53 to bind to  p21, but p53 was unable to be acetylated, indicating that proline-directed acetylation of p53 is a post-DNA binding event ( ,  ).	transcription
73372	4	336384	7	NULL	NULL	0	NULL	p53	GP		unable to be					acetylated	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_7_2782_s_29	16537920	Dornan et al. reported that site-specific acetylation of p53 was DNA dependent; deletion of the p53 proline repeat allows p53 to bind to  p21, but p53 was unable to be acetylated, indicating that proline-directed acetylation of p53 is a post-DNA binding event ( ,  ).	transcription
73373	5	336384	7	NULL	NULL	0	NULL	proline	AminoAcid		directs					p53	GP	acetylation of			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_7_2782_s_29	16537920	Dornan et al. reported that site-specific acetylation of p53 was DNA dependent; deletion of the p53 proline repeat allows p53 to bind to  p21, but p53 was unable to be acetylated, indicating that proline-directed acetylation of p53 is a post-DNA binding event ( ,  ).	transcription
73374	6	336384	7	NULL	NULL	0	NULL	statement 5	Process		is a type of					post-DNA binding event	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_7_2782_s_29	16537920	Dornan et al. reported that site-specific acetylation of p53 was DNA dependent; deletion of the p53 proline repeat allows p53 to bind to  p21, but p53 was unable to be acetylated, indicating that proline-directed acetylation of p53 is a post-DNA binding event ( ,  ).	transcription
73375	7	336384	7	NULL	NULL	0	NULL	statement 4	Process		indicates					statement 6	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_7_2782_s_29	16537920	Dornan et al. reported that site-specific acetylation of p53 was DNA dependent; deletion of the p53 proline repeat allows p53 to bind to  p21, but p53 was unable to be acetylated, indicating that proline-directed acetylation of p53 is a post-DNA binding event ( ,  ).	transcription
73376	1	336385	7	NULL	NULL	NULL	NULL	antiacetylated p53 antibody	GP		bind					p53 protein	GP	crosslinked			NULL		NULL	NULL	NULL	NULL	gw70_pnas_101_8_2259_s_133	14982997	Interestingly, although the antiacetylated p53 antibody only immunoprecipitated a small fraction of the total crosslinked p53 protein ( Fig. 3 B, lane 8 vs. 7), the p53 bound to the p21 promoter was enriched about 3-fold in acetylated p53 relative to total p53 ( Fig. 3 C).	transcription
73377	2	336385	7	NULL	NULL	0	NULL	p53	GP		bind					p21	GP			promoter	NULL		0	NULL	NULL	NULL	gw70_pnas_101_8_2259_s_133	14982997	Interestingly, although the antiacetylated p53 antibody only immunoprecipitated a small fraction of the total crosslinked p53 protein ( Fig. 3 B, lane 8 vs. 7), the p53 bound to the p21 promoter was enriched about 3-fold in acetylated p53 relative to total p53 ( Fig. 3 C).	transcription
73378	1	336386	7	NULL	NULL	0	NULL	acetyl-CoA	Chemical		promotes					p53	GP	weak;;acetylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_15_13431_s_179	12499368	Using the basal p300-acetylation reaction where acetyl-CoA promotes weak p53 acetylation (Fig.  4 C,  lane 3 versus lane 2), experiments demonstrated a stimulation of p53 acetylation by p300 upon titration of an excess of consensus site oligonucleotide DNA ( pG DNA; Fig.  5 A,  lanes 5-8 versus lane 4).	transcription
73379	2	336386	7	NULL	NULL	0	NULL	p300	GP		stimulates					p53	GP	acetylation of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_278_15_13431_s_179	12499368	Using the basal p300-acetylation reaction where acetyl-CoA promotes weak p53 acetylation (Fig.  4 C,  lane 3 versus lane 2), experiments demonstrated a stimulation of p53 acetylation by p300 upon titration of an excess of consensus site oligonucleotide DNA ( pG DNA; Fig.  5 A,  lanes 5-8 versus lane 4).	transcription
73380	1	336387	7	NULL	NULL	0	NULL	histones	GP		substrate for					PCAF	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_97_21_11303_s_13	11027331	Although histones are physiologically relevant substrates for PCAF, PCAF also acetylates transcriptional activators p53 ( 6,  7) and MyoD ( 8), as originally demonstrated by p300 acetylase ( 9), and stimulates DNA binding.	transcription
73381	2	336387	7	NULL	NULL	0	NULL	PCAF	GP		acetylates					p53	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_97_21_11303_s_13	11027331	Although histones are physiologically relevant substrates for PCAF, PCAF also acetylates transcriptional activators p53 ( 6,  7) and MyoD ( 8), as originally demonstrated by p300 acetylase ( 9), and stimulates DNA binding.	transcription
73382	3	336387	7	NULL	NULL	0	NULL	PCAF	GP		acetylates					MyoD	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_97_21_11303_s_13	11027331	Although histones are physiologically relevant substrates for PCAF, PCAF also acetylates transcriptional activators p53 ( 6,  7) and MyoD ( 8), as originally demonstrated by p300 acetylase ( 9), and stimulates DNA binding.	transcription
73383	4	336387	7	NULL	NULL	0	NULL	p53	GP		bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_pnas_97_21_11303_s_13	11027331	Although histones are physiologically relevant substrates for PCAF, PCAF also acetylates transcriptional activators p53 ( 6,  7) and MyoD ( 8), as originally demonstrated by p300 acetylase ( 9), and stimulates DNA binding.	transcription
73384	5	336387	7	NULL	NULL	0	NULL	MyoD	GP		bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_pnas_97_21_11303_s_13	11027331	Although histones are physiologically relevant substrates for PCAF, PCAF also acetylates transcriptional activators p53 ( 6,  7) and MyoD ( 8), as originally demonstrated by p300 acetylase ( 9), and stimulates DNA binding.	transcription
73385	6	336387	7	NULL	NULL	NULL	NULL	statement 2	Process		stimulate					statement 4	Process				NULL		NULL	NULL	NULL	NULL	gw60_pnas_97_21_11303_s_13	11027331	Although histones are physiologically relevant substrates for PCAF, PCAF also acetylates transcriptional activators p53 ( 6,  7) and MyoD ( 8), as originally demonstrated by p300 acetylase ( 9), and stimulates DNA binding.	transcription
73386	7	336387	7	NULL	NULL	0	NULL	statement 3	Process		stimulate					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_97_21_11303_s_13	11027331	Although histones are physiologically relevant substrates for PCAF, PCAF also acetylates transcriptional activators p53 ( 6,  7) and MyoD ( 8), as originally demonstrated by p300 acetylase ( 9), and stimulates DNA binding.	transcription
73387	8	336387	7	NULL	NULL	0	NULL	p53	GP		is a type of					transcriptional activator	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_97_21_11303_s_13	11027331	Although histones are physiologically relevant substrates for PCAF, PCAF also acetylates transcriptional activators p53 ( 6,  7) and MyoD ( 8), as originally demonstrated by p300 acetylase ( 9), and stimulates DNA binding.	transcription
73388	9	336387	7	NULL	NULL	0	NULL	MyoD	GP		is a type of					transcriptional coactivator	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_97_21_11303_s_13	11027331	Although histones are physiologically relevant substrates for PCAF, PCAF also acetylates transcriptional activators p53 ( 6,  7) and MyoD ( 8), as originally demonstrated by p300 acetylase ( 9), and stimulates DNA binding.	transcription
73389	1	336388	7	NULL	NULL	0	NULL	CBP/p300	GP		acetylates		directly			GATA-1	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_19_7300_s_337	10982847	Moreover, CBP/p300 directly acetylates transcription factors such as GATA-1 ( 6) and p53 ( 21).	transcription
73390	2	336388	7	NULL	NULL	0	NULL	CBP/p300	GP		acetylates		directly			p53	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_19_7300_s_337	10982847	Moreover, CBP/p300 directly acetylates transcription factors such as GATA-1 ( 6) and p53 ( 21).	transcription
73391	3	336388	7	NULL	NULL	0	NULL	GATA-1	GP		is a type of					transcription factor	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_19_7300_s_337	10982847	Moreover, CBP/p300 directly acetylates transcription factors such as GATA-1 ( 6) and p53 ( 21).	transcription
73392	4	336388	7	NULL	NULL	0	NULL	p53	GP		is a type of					transcription factor	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_19_7300_s_337	10982847	Moreover, CBP/p300 directly acetylates transcription factors such as GATA-1 ( 6) and p53 ( 21).	transcription
73393	1	336389	7	NULL	NULL	0	NULL	p300	GP		acetylates					p53	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_97_23_12547_s_2	11070080	p300 acetylates and activates the tumor suppressor p53 after DNA damage.	transcription
73394	2	336389	7	NULL	NULL	0	NULL	statement 1	Process		activates					p53	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_97_23_12547_s_2	11070080	p300 acetylates and activates the tumor suppressor p53 after DNA damage.	transcription
73395	3	336389	7	NULL	NULL	0	NULL	statement 2	Process		occur after					DNA damage	Process				NULL		0	NULL	NULL	NULL	gw60_pnas_97_23_12547_s_2	11070080	p300 acetylates and activates the tumor suppressor p53 after DNA damage.	transcription
73396	4	336389	7	NULL	NULL	0	NULL	p53	GP		is a type of					tumor suppressor	GP				NULL		0	NULL	NULL	NULL	gw60_pnas_97_23_12547_s_2	11070080	p300 acetylates and activates the tumor suppressor p53 after DNA damage.	transcription
73397	1	336390	7	NULL	NULL	0	NULL	p300	GP		acetylates					p53	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_26_24315_s_77	15851483	Expression of MLL Fusions Decreases p53 Acetylation by p300 in Response to Ionizing Radiation -- p300 is an important co-activator of p53 transcriptional activity that acetylates several critical lysine residues on the p53 C terminus ( ).	transcription
73398	2	336390	7	NULL	NULL	0	NULL	MLL Fusions	GP	expression of	decrease					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_26_24315_s_77	15851483	Expression of MLL Fusions Decreases p53 Acetylation by p300 in Response to Ionizing Radiation -- p300 is an important co-activator of p53 transcriptional activity that acetylates several critical lysine residues on the p53 C terminus ( ).	transcription
73399	3	336390	7	NULL	NULL	0	NULL	statement 2	Process		in response to					ionizing radiation	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_26_24315_s_77	15851483	Expression of MLL Fusions Decreases p53 Acetylation by p300 in Response to Ionizing Radiation -- p300 is an important co-activator of p53 transcriptional activity that acetylates several critical lysine residues on the p53 C terminus ( ).	transcription
73400	4	336390	7	NULL	NULL	0	NULL	p300	GP		coactivator of					p53	GP	transcriptional activity of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_26_24315_s_77	15851483	Expression of MLL Fusions Decreases p53 Acetylation by p300 in Response to Ionizing Radiation -- p300 is an important co-activator of p53 transcriptional activity that acetylates several critical lysine residues on the p53 C terminus ( ).	transcription
73401	5	336390	7	NULL	NULL	0	NULL	p300	GP		acetylates					p53	GP		lysine residues on C terminus		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_280_26_24315_s_77	15851483	Expression of MLL Fusions Decreases p53 Acetylation by p300 in Response to Ionizing Radiation -- p300 is an important co-activator of p53 transcriptional activity that acetylates several critical lysine residues on the p53 C terminus ( ).	transcription
73402	1	336391	7	NULL	NULL	0	NULL	p53	GP	acetylated	bind					TRRAP	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_28_25401_s_250	12738767	In this context, Barlev  et al.  ( ) showed that acetylated  p53 binds more tightly to the transcriptional cofactors TRRAP and CBP than  nonacetylated p53, although acetylated and nonacetylated p53 bind to the p21  promoter in the same manner.	transcription
73403	2	336391	7	NULL	NULL	0	NULL	p53	GP	acetylated	bind					CBP	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_28_25401_s_250	12738767	In this context, Barlev  et al.  ( ) showed that acetylated  p53 binds more tightly to the transcriptional cofactors TRRAP and CBP than  nonacetylated p53, although acetylated and nonacetylated p53 bind to the p21  promoter in the same manner.	transcription
73404	3	336391	7	NULL	NULL	0	NULL	p53	GP	nonacetylated	bind					TRRAP	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_28_25401_s_250	12738767	In this context, Barlev  et al.  ( ) showed that acetylated  p53 binds more tightly to the transcriptional cofactors TRRAP and CBP than  nonacetylated p53, although acetylated and nonacetylated p53 bind to the p21  promoter in the same manner.	transcription
73405	4	336391	7	NULL	NULL	0	NULL	p53	GP	nonacetylated	bind					CBP	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_28_25401_s_250	12738767	In this context, Barlev  et al.  ( ) showed that acetylated  p53 binds more tightly to the transcriptional cofactors TRRAP and CBP than  nonacetylated p53, although acetylated and nonacetylated p53 bind to the p21  promoter in the same manner.	transcription
73406	5	336391	7	NULL	NULL	0	NULL	statement 1	Process	binding of	is tighter than					statement 3	Process	binding of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_28_25401_s_250	12738767	In this context, Barlev  et al.  ( ) showed that acetylated  p53 binds more tightly to the transcriptional cofactors TRRAP and CBP than  nonacetylated p53, although acetylated and nonacetylated p53 bind to the p21  promoter in the same manner.	transcription
73407	6	336391	7	NULL	NULL	0	NULL	statement 2	Process	binding of	is tighter than					statement 4	Process	binding of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_28_25401_s_250	12738767	In this context, Barlev  et al.  ( ) showed that acetylated  p53 binds more tightly to the transcriptional cofactors TRRAP and CBP than  nonacetylated p53, although acetylated and nonacetylated p53 bind to the p21  promoter in the same manner.	transcription
73408	7	336391	7	NULL	NULL	NULL	NULL	p53	GP	acetylated	bind					p21	GP			promoter	NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_278_28_25401_s_250	12738767	In this context, Barlev  et al.  ( ) showed that acetylated  p53 binds more tightly to the transcriptional cofactors TRRAP and CBP than  nonacetylated p53, although acetylated and nonacetylated p53 bind to the p21  promoter in the same manner.	transcription
73409	8	336391	7	NULL	NULL	0	NULL	p53	GP	nonacetylated	bind					p21	GP			promoter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_28_25401_s_250	12738767	In this context, Barlev  et al.  ( ) showed that acetylated  p53 binds more tightly to the transcriptional cofactors TRRAP and CBP than  nonacetylated p53, although acetylated and nonacetylated p53 bind to the p21  promoter in the same manner.	transcription
73410	1	336392	7	NULL	NULL	NULL	NULL	CBP		mutant;;purified	is defective in			acetylase domain;;L160K/C161L		acetyltransferase activity	Process				NULL		NULL	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_1_118_s_67	12147236	As purified CBP acetylase domain that contains point mutations (L160K/C161L) and is defective in acetyltransferase activity stimulated p53 DNA binding activity as well as the wild-type acetyltransferase domain (data not shown), we examined the effect of these domains on p53 DNA binding.	transcription
73411	2	336392	7	NULL	NULL	0	NULL	p53	GP		bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_1_118_s_67	12147236	As purified CBP acetylase domain that contains point mutations (L160K/C161L) and is defective in acetyltransferase activity stimulated p53 DNA binding activity as well as the wild-type acetyltransferase domain (data not shown), we examined the effect of these domains on p53 DNA binding.	transcription
73412	3	336392	7	NULL	NULL	0	NULL	statement 1	Process		stimulate					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_1_118_s_67	12147236	As purified CBP acetylase domain that contains point mutations (L160K/C161L) and is defective in acetyltransferase activity stimulated p53 DNA binding activity as well as the wild-type acetyltransferase domain (data not shown), we examined the effect of these domains on p53 DNA binding.	transcription
73413	4	336392	7	NULL	NULL	0	NULL	CBP	GP	wild-type	stimulate			acetyltransferase domain		statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_biochmbiophyrescomm_296_1_118_s_67	12147236	As purified CBP acetylase domain that contains point mutations (L160K/C161L) and is defective in acetyltransferase activity stimulated p53 DNA binding activity as well as the wild-type acetyltransferase domain (data not shown), we examined the effect of these domains on p53 DNA binding.	transcription
73414	1	336393	7	NULL	NULL	0	NULL	UV irradiation	PhysicalPhenomenon		acetylates					p53	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_27_24594_s_181	12716906	This pattern of changes  in p53 acetylation is different from that induced by UV irradiation, which  acetylates p53 at all three sites in ECs  ( Fig. 1 B).	transcription
73415	2	336393	7	NULL	NULL	0	NULL	statement 1	Process		occur in					ECs	Cell				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_27_24594_s_181	12716906	This pattern of changes  in p53 acetylation is different from that induced by UV irradiation, which  acetylates p53 at all three sites in ECs  ( Fig. 1 B).	transcription
73416	1	336394	7	NULL	NULL	0	NULL	p53	GP		interacts with		directly			p300	GP				NULL		0	NULL	NULL	NULL	gw60_molcell_10_5_1213_s_205	12453427	p53 interacts directly with p300 that acetylates two specific lysine residues within p53 (lysine residues 373 and 382)  (Gu and Roeder, 1997  ).	transcription
73417	2	336394	7	NULL	NULL	0	NULL	p300	GP		acetylates					p53	GP		lysine residues 373 and 382		NULL		0	NULL	NULL	NULL	gw60_molcell_10_5_1213_s_205	12453427	p53 interacts directly with p300 that acetylates two specific lysine residues within p53 (lysine residues 373 and 382)  (Gu and Roeder, 1997  ).	transcription
73418	1	336395	7	NULL	NULL	0	NULL	PCAF	GP		acetylates					p53	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_2_1202_s_99	9891054	[[            Since PCAF acetylates p53 ]] within a specific domain, we wanted to determine whether a stable interaction could be detected between PCAF and p53.	transcription
73419	1	336396	7	NULL	NULL	0	NULL	p53	GP		associate with					U1 snRNA gene	GP	endogenous		promoter	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_8_3247_s_178	15798209	Together, these data indicate that p53 associates with the endogenous U1 and U2 snRNA gene promoters prior to genotypic stress and UV light stimulates p53 association with these promoters, although the apparent proportion of p53 that is acetylated decreases.	transcription
73420	2	336396	7	NULL	NULL	0	NULL	p53	GP		associate with					U2 snRNA gene	GP	endogenous		promoter	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_8_3247_s_178	15798209	Together, these data indicate that p53 associates with the endogenous U1 and U2 snRNA gene promoters prior to genotypic stress and UV light stimulates p53 association with these promoters, although the apparent proportion of p53 that is acetylated decreases.	transcription
73421	3	336396	7	NULL	NULL	0	NULL	statement 1	Process		prior to					genotypic stress	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_8_3247_s_178	15798209	Together, these data indicate that p53 associates with the endogenous U1 and U2 snRNA gene promoters prior to genotypic stress and UV light stimulates p53 association with these promoters, although the apparent proportion of p53 that is acetylated decreases.	transcription
73422	4	336396	7	NULL	NULL	0	NULL	statement 2	Process		prior to					genotypic stress	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_8_3247_s_178	15798209	Together, these data indicate that p53 associates with the endogenous U1 and U2 snRNA gene promoters prior to genotypic stress and UV light stimulates p53 association with these promoters, although the apparent proportion of p53 that is acetylated decreases.	transcription
73423	5	336396	7	NULL	NULL	0	NULL	UVlight	PhysicalPhenomenon		stimulate					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_8_3247_s_178	15798209	Together, these data indicate that p53 associates with the endogenous U1 and U2 snRNA gene promoters prior to genotypic stress and UV light stimulates p53 association with these promoters, although the apparent proportion of p53 that is acetylated decreases.	transcription
73424	6	336396	7	NULL	NULL	0	NULL	UVlight	PhysicalPhenomenon		stimulate					statement 2	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_8_3247_s_178	15798209	Together, these data indicate that p53 associates with the endogenous U1 and U2 snRNA gene promoters prior to genotypic stress and UV light stimulates p53 association with these promoters, although the apparent proportion of p53 that is acetylated decreases.	transcription
73425	7	336396	7	NULL	NULL	0	NULL	statement 1	Process		decrease					p53	GP	acetylated			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_8_3247_s_178	15798209	Together, these data indicate that p53 associates with the endogenous U1 and U2 snRNA gene promoters prior to genotypic stress and UV light stimulates p53 association with these promoters, although the apparent proportion of p53 that is acetylated decreases.	transcription
73426	8	336396	7	NULL	NULL	0	NULL	statement 2	Process		decrease					p53	GP	acetylated			NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_8_3247_s_178	15798209	Together, these data indicate that p53 associates with the endogenous U1 and U2 snRNA gene promoters prior to genotypic stress and UV light stimulates p53 association with these promoters, although the apparent proportion of p53 that is acetylated decreases.	transcription
73427	1	336397	7	NULL	NULL	0	NULL	HDM2	GP		inhibit					p53	GP	acetylation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_25_16943_s_228	16624812	In contrast, HDM2 inhibits the acetylation of p53, and under-acetylated p53 displays altered cell cycle regulation, reduced apoptosis, and altered promoter selectivity without changing binding of p53 to the promoter regions that were examined.	transcription
73428	2	336397	7	NULL	NULL	0	NULL	p53	GP	under-acetylated	display					cell cycle regulation	Process	altered			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_25_16943_s_228	16624812	In contrast, HDM2 inhibits the acetylation of p53, and under-acetylated p53 displays altered cell cycle regulation, reduced apoptosis, and altered promoter selectivity without changing binding of p53 to the promoter regions that were examined.	transcription
73429	3	336397	7	NULL	NULL	0	NULL	p53	GP	under-acetylated	display					apoptosis	Process	reduced			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_25_16943_s_228	16624812	In contrast, HDM2 inhibits the acetylation of p53, and under-acetylated p53 displays altered cell cycle regulation, reduced apoptosis, and altered promoter selectivity without changing binding of p53 to the promoter regions that were examined.	transcription
73430	4	336397	7	NULL	NULL	0	NULL	p53	GP	under-acetylated	display							altered selectivity of		promoter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_25_16943_s_228	16624812	In contrast, HDM2 inhibits the acetylation of p53, and under-acetylated p53 displays altered cell cycle regulation, reduced apoptosis, and altered promoter selectivity without changing binding of p53 to the promoter regions that were examined.	transcription
73431	5	336397	7	NULL	NULL	0	NULL	p53	GP		bind									promoter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_25_16943_s_228	16624812	In contrast, HDM2 inhibits the acetylation of p53, and under-acetylated p53 displays altered cell cycle regulation, reduced apoptosis, and altered promoter selectivity without changing binding of p53 to the promoter regions that were examined.	transcription
73432	6	336397	7	NULL	NULL	0	NULL	statement 2	Process		without changing					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_25_16943_s_228	16624812	In contrast, HDM2 inhibits the acetylation of p53, and under-acetylated p53 displays altered cell cycle regulation, reduced apoptosis, and altered promoter selectivity without changing binding of p53 to the promoter regions that were examined.	transcription
73433	7	336397	7	NULL	NULL	0	NULL	statement 3	Process		without changing					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_25_16943_s_228	16624812	In contrast, HDM2 inhibits the acetylation of p53, and under-acetylated p53 displays altered cell cycle regulation, reduced apoptosis, and altered promoter selectivity without changing binding of p53 to the promoter regions that were examined.	transcription
73434	8	336397	7	NULL	NULL	0	NULL	statement 4	Process		without changing					statement 5	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_25_16943_s_228	16624812	In contrast, HDM2 inhibits the acetylation of p53, and under-acetylated p53 displays altered cell cycle regulation, reduced apoptosis, and altered promoter selectivity without changing binding of p53 to the promoter regions that were examined.	transcription
73435	1	336398	7	NULL	NULL	0	NULL	p53	GP		recruit					p300/CBP	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_19_17557_s_40	12609999	Therefore, our data suggest that the amount of p300/CBP recruited by p53 and the extent of acetylated histones bound to the proximal promoter can in part explain the differential transcriptional activity among wild-type p53 and various p53 mutants.	transcription
73436	2	336398	7	NULL	NULL	0	NULL	histones	GP	acetylated	bind									proximal promoter	NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_19_17557_s_40	12609999	Therefore, our data suggest that the amount of p300/CBP recruited by p53 and the extent of acetylated histones bound to the proximal promoter can in part explain the differential transcriptional activity among wild-type p53 and various p53 mutants.	transcription
73437	1	336399	7	NULL	NULL	0	NULL	SIRT1 	GP		deacetylate					p53	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_100_19_10794_s_155	12960381	However, p53 was still clearly more acetylated in SIRT1deltaex4/deltaex4, than in SIRT1+/+ and SIRT1+/deltaex4 MEFs ( Fig. 3 B), providing evidence that SIRT1 deacetylation of p53 is not fully redundant with HDAC-mediated p53 deacetylation.	transcription
73438	2	336399	7	NULL	NULL	0	NULL	HDAC	GP		mediate					p53	GP	deacetylation of			NULL		0	NULL	NULL	NULL	gw70_pnas_100_19_10794_s_155	12960381	However, p53 was still clearly more acetylated in SIRT1deltaex4/deltaex4, than in SIRT1+/+ and SIRT1+/deltaex4 MEFs ( Fig. 3 B), providing evidence that SIRT1 deacetylation of p53 is not fully redundant with HDAC-mediated p53 deacetylation.	transcription
73439	3	336399	7	NULL	NULL	0	NULL	p53	GP	acetylation of	occur in					SIRT1deltaex4/deltaex4 MEF	Cell				NULL		0	NULL	NULL	NULL	gw70_pnas_100_19_10794_s_155	12960381	However, p53 was still clearly more acetylated in SIRT1deltaex4/deltaex4, than in SIRT1+/+ and SIRT1+/deltaex4 MEFs ( Fig. 3 B), providing evidence that SIRT1 deacetylation of p53 is not fully redundant with HDAC-mediated p53 deacetylation.	transcription
73440	4	336399	7	NULL	NULL	0	NULL	p53	GP	acetylation of	occur in					SIRT1+/+ MEF	Cell				NULL		0	NULL	NULL	NULL	gw70_pnas_100_19_10794_s_155	12960381	However, p53 was still clearly more acetylated in SIRT1deltaex4/deltaex4, than in SIRT1+/+ and SIRT1+/deltaex4 MEFs ( Fig. 3 B), providing evidence that SIRT1 deacetylation of p53 is not fully redundant with HDAC-mediated p53 deacetylation.	transcription
73441	5	336399	7	NULL	NULL	NULL	NULL	p53	GP	acetylation of	occur in					SIRT1+/deltaex4 MEF	Cell				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_19_10794_s_155	12960381	However, p53 was still clearly more acetylated in SIRT1deltaex4/deltaex4, than in SIRT1+/+ and SIRT1+/deltaex4 MEFs ( Fig. 3 B), providing evidence that SIRT1 deacetylation of p53 is not fully redundant with HDAC-mediated p53 deacetylation.	transcription
73442	6	336399	7	NULL	NULL	NULL	NULL	statement 3	Process	acetylation of	is more than					statement 4	Process	acetylation of			NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_19_10794_s_155	12960381	However, p53 was still clearly more acetylated in SIRT1deltaex4/deltaex4, than in SIRT1+/+ and SIRT1+/deltaex4 MEFs ( Fig. 3 B), providing evidence that SIRT1 deacetylation of p53 is not fully redundant with HDAC-mediated p53 deacetylation.	transcription
73443	7	336399	7	NULL	NULL	0	NULL	statement 3	Process	acetylation of	is more than					statement 5	Process	acetylation of			NULL		0	NULL	NULL	NULL	gw70_pnas_100_19_10794_s_155	12960381	However, p53 was still clearly more acetylated in SIRT1deltaex4/deltaex4, than in SIRT1+/+ and SIRT1+/deltaex4 MEFs ( Fig. 3 B), providing evidence that SIRT1 deacetylation of p53 is not fully redundant with HDAC-mediated p53 deacetylation.	transcription
73444	8	336399	7	NULL	NULL	NULL	NULL	statement 1	Process		 not redundant with		fully			statement 2	Process				NULL		NULL	NULL	NULL	NULL	gw70_pnas_100_19_10794_s_155	12960381	However, p53 was still clearly more acetylated in SIRT1deltaex4/deltaex4, than in SIRT1+/+ and SIRT1+/deltaex4 MEFs ( Fig. 3 B), providing evidence that SIRT1 deacetylation of p53 is not fully redundant with HDAC-mediated p53 deacetylation.	transcription
73445	1	336400	7	NULL	NULL	NULL	NULL	p300	GP		acetylate					p53	GP		C terminus		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_21_17_5979_s_317	11486036	This finding is reminiscent of acetylation of p53 by p300, in which the N terminus of p53 interacts with CBP ( 19,  41) while the region acetylated by p300 is at the C terminus of p53 ( 18).	transcription
73446	2	336400	7	NULL	NULL	0	NULL	p53	GP		interacts with			N terminus		CBP	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_17_5979_s_317	11486036	This finding is reminiscent of acetylation of p53 by p300, in which the N terminus of p53 interacts with CBP ( 19,  41) while the region acetylated by p300 is at the C terminus of p53 ( 18).	transcription
73447	1	336401	7	NULL	NULL	0	NULL	p300	GP		acetylate					p53	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_15_5540_s_4	10891493	It was shown recently that p53 is acetylated by transcriptional coactivators p300, CREB bidning protein (CBP), and PCAF and that acetylation of p53 by these proteins enhances p53 sequence-specific DNA binding.	transcription
73448	2	336401	7	NULL	NULL	0	NULL	CBP	GP		acetylate					p53	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_15_5540_s_4	10891493	It was shown recently that p53 is acetylated by transcriptional coactivators p300, CREB bidning protein (CBP), and PCAF and that acetylation of p53 by these proteins enhances p53 sequence-specific DNA binding.	transcription
73449	3	336401	7	NULL	NULL	0	NULL	PCAF	GP		acetylate					p53	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_15_5540_s_4	10891493	It was shown recently that p53 is acetylated by transcriptional coactivators p300, CREB bidning protein (CBP), and PCAF and that acetylation of p53 by these proteins enhances p53 sequence-specific DNA binding.	transcription
73450	4	336401	7	NULL	NULL	NULL	NULL	p53	GP		bind		sequence-specific			DNA	NucleicAcid				NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5540_s_4	10891493	It was shown recently that p53 is acetylated by transcriptional coactivators p300, CREB bidning protein (CBP), and PCAF and that acetylation of p53 by these proteins enhances p53 sequence-specific DNA binding.	transcription
73451	5	336401	7	NULL	NULL	0	NULL	statement 1	Process		enhance					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_15_5540_s_4	10891493	It was shown recently that p53 is acetylated by transcriptional coactivators p300, CREB bidning protein (CBP), and PCAF and that acetylation of p53 by these proteins enhances p53 sequence-specific DNA binding.	transcription
73452	6	336401	7	NULL	NULL	0	NULL	statement 2	Process		enhance					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_15_5540_s_4	10891493	It was shown recently that p53 is acetylated by transcriptional coactivators p300, CREB bidning protein (CBP), and PCAF and that acetylation of p53 by these proteins enhances p53 sequence-specific DNA binding.	transcription
73453	7	336401	7	NULL	NULL	0	NULL	statement 3	Process		enhance					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_15_5540_s_4	10891493	It was shown recently that p53 is acetylated by transcriptional coactivators p300, CREB bidning protein (CBP), and PCAF and that acetylation of p53 by these proteins enhances p53 sequence-specific DNA binding.	transcription
73454	8	336401	7	NULL	NULL	0	NULL	CBP	GP		is					CREB bidning protein	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_15_5540_s_4	10891493	It was shown recently that p53 is acetylated by transcriptional coactivators p300, CREB bidning protein (CBP), and PCAF and that acetylation of p53 by these proteins enhances p53 sequence-specific DNA binding.	transcription
73455	9	336401	7	NULL	NULL	0	NULL	p300	GP		is a type of					transcriptional coactivator	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_15_5540_s_4	10891493	It was shown recently that p53 is acetylated by transcriptional coactivators p300, CREB bidning protein (CBP), and PCAF and that acetylation of p53 by these proteins enhances p53 sequence-specific DNA binding.	transcription
73456	10	336401	7	NULL	NULL	0	NULL	CBP	GP		is a type of					transcriptional coactivator	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_15_5540_s_4	10891493	It was shown recently that p53 is acetylated by transcriptional coactivators p300, CREB bidning protein (CBP), and PCAF and that acetylation of p53 by these proteins enhances p53 sequence-specific DNA binding.	transcription
73457	11	336401	7	NULL	NULL	0	NULL	PCAF	GP		is a type of					transcriptional coactivator	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_15_5540_s_4	10891493	It was shown recently that p53 is acetylated by transcriptional coactivators p300, CREB bidning protein (CBP), and PCAF and that acetylation of p53 by these proteins enhances p53 sequence-specific DNA binding.	transcription
73458	1	336402	7	NULL	NULL	0	NULL	ATM	GP		detect					genotoxic stress	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1552_2_47_s_178	11825686	So-called stress kinases (e.g. ATM, ATR, Chk2) which detect genotoxic stress and initiate signal transduction are in vivo kinases for specific p53 serine residues, while the histone acetyltransferases p300/CBP and PCAF (which at the same time are transcriptional coactivators) acetylate p53.	transcription
73459	2	336402	7	NULL	NULL	0	NULL	ATR	GP		detect					genotoxic stress	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1552_2_47_s_178	11825686	So-called stress kinases (e.g. ATM, ATR, Chk2) which detect genotoxic stress and initiate signal transduction are in vivo kinases for specific p53 serine residues, while the histone acetyltransferases p300/CBP and PCAF (which at the same time are transcriptional coactivators) acetylate p53.	transcription
73460	3	336402	7	NULL	NULL	0	NULL	Chk2	GP		detect					genotoxic stress	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1552_2_47_s_178	11825686	So-called stress kinases (e.g. ATM, ATR, Chk2) which detect genotoxic stress and initiate signal transduction are in vivo kinases for specific p53 serine residues, while the histone acetyltransferases p300/CBP and PCAF (which at the same time are transcriptional coactivators) acetylate p53.	transcription
73461	4	336402	7	NULL	NULL	0	NULL	statement 1	Process		initiate					signal transduction	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1552_2_47_s_178	11825686	So-called stress kinases (e.g. ATM, ATR, Chk2) which detect genotoxic stress and initiate signal transduction are in vivo kinases for specific p53 serine residues, while the histone acetyltransferases p300/CBP and PCAF (which at the same time are transcriptional coactivators) acetylate p53.	transcription
73462	5	336402	7	NULL	NULL	0	NULL	statement 2	Process		initiate					signal transduction	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1552_2_47_s_178	11825686	So-called stress kinases (e.g. ATM, ATR, Chk2) which detect genotoxic stress and initiate signal transduction are in vivo kinases for specific p53 serine residues, while the histone acetyltransferases p300/CBP and PCAF (which at the same time are transcriptional coactivators) acetylate p53.	transcription
73463	6	336402	7	NULL	NULL	0	NULL	statement 3	Process		initiate					signal transduction	Process				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1552_2_47_s_178	11825686	So-called stress kinases (e.g. ATM, ATR, Chk2) which detect genotoxic stress and initiate signal transduction are in vivo kinases for specific p53 serine residues, while the histone acetyltransferases p300/CBP and PCAF (which at the same time are transcriptional coactivators) acetylate p53.	transcription
73464	7	336402	7	NULL	NULL	NULL	NULL	ATM	GP		kinase for					p53	GP		serine residue		NULL	in vivo	NULL	NULL	NULL	NULL	gw60_biochimbiophysacta_1552_2_47_s_178	11825686	So-called stress kinases (e.g. ATM, ATR, Chk2) which detect genotoxic stress and initiate signal transduction are in vivo kinases for specific p53 serine residues, while the histone acetyltransferases p300/CBP and PCAF (which at the same time are transcriptional coactivators) acetylate p53.	transcription
73465	8	336402	7	NULL	NULL	0	NULL	ATR	GP		kinase for					p53	GP		serine residue		NULL	in vivo	0	NULL	NULL	NULL	gw60_biochimbiophysacta_1552_2_47_s_178	11825686	So-called stress kinases (e.g. ATM, ATR, Chk2) which detect genotoxic stress and initiate signal transduction are in vivo kinases for specific p53 serine residues, while the histone acetyltransferases p300/CBP and PCAF (which at the same time are transcriptional coactivators) acetylate p53.	transcription
73466	9	336402	7	NULL	NULL	0	NULL	Chk2	GP		kinase for					p53	GP		serine residue		NULL	in vivo	0	NULL	NULL	NULL	gw60_biochimbiophysacta_1552_2_47_s_178	11825686	So-called stress kinases (e.g. ATM, ATR, Chk2) which detect genotoxic stress and initiate signal transduction are in vivo kinases for specific p53 serine residues, while the histone acetyltransferases p300/CBP and PCAF (which at the same time are transcriptional coactivators) acetylate p53.	transcription
73467	10	336402	7	NULL	NULL	0	NULL	p300/CBP	GP		acetylate					p53	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1552_2_47_s_178	11825686	So-called stress kinases (e.g. ATM, ATR, Chk2) which detect genotoxic stress and initiate signal transduction are in vivo kinases for specific p53 serine residues, while the histone acetyltransferases p300/CBP and PCAF (which at the same time are transcriptional coactivators) acetylate p53.	transcription
73468	11	336402	7	NULL	NULL	0	NULL	PCAF	GP		acetylate					p53	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1552_2_47_s_178	11825686	So-called stress kinases (e.g. ATM, ATR, Chk2) which detect genotoxic stress and initiate signal transduction are in vivo kinases for specific p53 serine residues, while the histone acetyltransferases p300/CBP and PCAF (which at the same time are transcriptional coactivators) acetylate p53.	transcription
73469	12	336402	7	NULL	NULL	0	NULL	p300/CBP	GP		is a type of					histone acetyl transferases	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1552_2_47_s_178	11825686	So-called stress kinases (e.g. ATM, ATR, Chk2) which detect genotoxic stress and initiate signal transduction are in vivo kinases for specific p53 serine residues, while the histone acetyltransferases p300/CBP and PCAF (which at the same time are transcriptional coactivators) acetylate p53.	transcription
73470	13	336402	7	NULL	NULL	0	NULL	PCAF	GP		is a type of					histone acetyl transferases	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1552_2_47_s_178	11825686	So-called stress kinases (e.g. ATM, ATR, Chk2) which detect genotoxic stress and initiate signal transduction are in vivo kinases for specific p53 serine residues, while the histone acetyltransferases p300/CBP and PCAF (which at the same time are transcriptional coactivators) acetylate p53.	transcription
73471	14	336402	7	NULL	NULL	0	NULL	ATM	GP		is a type of					stress kinases	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1552_2_47_s_178	11825686	So-called stress kinases (e.g. ATM, ATR, Chk2) which detect genotoxic stress and initiate signal transduction are in vivo kinases for specific p53 serine residues, while the histone acetyltransferases p300/CBP and PCAF (which at the same time are transcriptional coactivators) acetylate p53.	transcription
73472	15	336402	7	NULL	NULL	0	NULL	ATR	GP		is a type of					stress kinases	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1552_2_47_s_178	11825686	So-called stress kinases (e.g. ATM, ATR, Chk2) which detect genotoxic stress and initiate signal transduction are in vivo kinases for specific p53 serine residues, while the histone acetyltransferases p300/CBP and PCAF (which at the same time are transcriptional coactivators) acetylate p53.	transcription
73473	16	336402	7	NULL	NULL	0	NULL	Chk2	GP		is a type of					stress kinases	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1552_2_47_s_178	11825686	So-called stress kinases (e.g. ATM, ATR, Chk2) which detect genotoxic stress and initiate signal transduction are in vivo kinases for specific p53 serine residues, while the histone acetyltransferases p300/CBP and PCAF (which at the same time are transcriptional coactivators) acetylate p53.	transcription
73474	17	336402	7	NULL	NULL	0	NULL	p300/CBP	GP		is a type of					transcriptional coactivators	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1552_2_47_s_178	11825686	So-called stress kinases (e.g. ATM, ATR, Chk2) which detect genotoxic stress and initiate signal transduction are in vivo kinases for specific p53 serine residues, while the histone acetyltransferases p300/CBP and PCAF (which at the same time are transcriptional coactivators) acetylate p53.	transcription
73475	18	336402	7	NULL	NULL	0	NULL	PCAF	GP		is a type of					transcriptional coactivator	GP				NULL		0	NULL	NULL	NULL	gw60_biochimbiophysacta_1552_2_47_s_178	11825686	So-called stress kinases (e.g. ATM, ATR, Chk2) which detect genotoxic stress and initiate signal transduction are in vivo kinases for specific p53 serine residues, while the histone acetyltransferases p300/CBP and PCAF (which at the same time are transcriptional coactivators) acetylate p53.	transcription
73476	1	336403	7	NULL	NULL	0	NULL	p300	GP		bind					p21	GP			promoter	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_7_2782_s_225	16537920	p53 acetylated at K373/382 is required for recruitment of p300 to the  p21 promoter.	transcription
73477	2	336403	7	NULL	NULL	0	NULL	p53	GP	acetylated	required for			K373/382		statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_26_7_2782_s_225	16537920	p53 acetylated at K373/382 is required for recruitment of p300 to the  p21 promoter.	transcription
73478	1	336404	7	NULL	NULL	NULL	NULL	p300/CREB-binding protein	GP		acetylate					p53	GP		lysine		NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_3_1394_s_3	16291740	Upon p53 activation, however, these lysines become acetylated by p300/CREB-binding protein.	transcription
73479	2	336404	7	NULL	NULL	0	NULL	statement 1	Process		occur upon					p53	GP	activation of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_3_1394_s_3	16291740	Upon p53 activation, however, these lysines become acetylated by p300/CREB-binding protein.	transcription
73480	1	336405	7	NULL	NULL	NULL	NULL	p300	GP		acetylate					p53	GP		Lys-373;;Lys-382		NULL		NULL	NULL	NULL	NULL	gw60_molcellbiol_20_15_5540_s_182	10891493	p53 is acetylated by transcriptional coactivator p300 at Lys-373 and Lys-382 and by PCAF at Lys-320.	transcription
73481	2	336405	7	NULL	NULL	0	NULL	PCAF	GP		acetylate					p53	GP		Lys-320		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_15_5540_s_182	10891493	p53 is acetylated by transcriptional coactivator p300 at Lys-373 and Lys-382 and by PCAF at Lys-320.	transcription
73482	3	336405	7	NULL	NULL	0	NULL	p300	GP		is a type of					transcriptional coactivator	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_20_15_5540_s_182	10891493	p53 is acetylated by transcriptional coactivator p300 at Lys-373 and Lys-382 and by PCAF at Lys-320.	transcription
73483	1	336406	7	NULL	NULL	NULL	NULL	p53	GP		bind					p21	GP			 promoter	NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_2014_s_481	15713654	In support of our model, recent studies have demonstrated that p53 target gene expression requires more than just p53 binding: p53 first binds to the p21 promoter and recruits p300, which then acetylates the p21 proximal promoter and cooperates with p53 to induce p21 ( ,  ).	transcription
73484	2	336406	7	NULL	NULL	NULL	NULL	statement 1	GP		recruit					p300	GP				NULL		NULL	NULL	NULL	NULL	gw70_molcellbiol_25_5_2014_s_481	15713654	In support of our model, recent studies have demonstrated that p53 target gene expression requires more than just p53 binding: p53 first binds to the p21 promoter and recruits p300, which then acetylates the p21 proximal promoter and cooperates with p53 to induce p21 ( ,  ).	transcription
73485	3	336406	7	NULL	NULL	0	NULL	p300	GP		acetylate					p21	GP			proximal promoter	NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_5_2014_s_481	15713654	In support of our model, recent studies have demonstrated that p53 target gene expression requires more than just p53 binding: p53 first binds to the p21 promoter and recruits p300, which then acetylates the p21 proximal promoter and cooperates with p53 to induce p21 ( ,  ).	transcription
73486	4	336406	7	NULL	NULL	0	NULL	p53	GP		induce					p21	GP				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_5_2014_s_481	15713654	In support of our model, recent studies have demonstrated that p53 target gene expression requires more than just p53 binding: p53 first binds to the p21 promoter and recruits p300, which then acetylates the p21 proximal promoter and cooperates with p53 to induce p21 ( ,  ).	transcription
73487	5	336406	7	NULL	NULL	0	NULL	statement 3	Process		cooperates with					statement 4	Process				NULL		0	NULL	NULL	NULL	gw70_molcellbiol_25_5_2014_s_481	15713654	In support of our model, recent studies have demonstrated that p53 target gene expression requires more than just p53 binding: p53 first binds to the p21 promoter and recruits p300, which then acetylates the p21 proximal promoter and cooperates with p53 to induce p21 ( ,  ).	transcription
73488	1	336407	7	NULL	NULL	0	NULL	PCAF	GP		acetylates		specifically			p53	GP		K320		NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_2_1202_s_169	9891054	Our observations that PCAF specifically acetylates p53 at K320, that this acetylation stimulates p53's DNA binding in vitro, and that alteration of this residue partially lowers p53 transcriptional activity in vivo raised the question of whether the acetylation occurs in vivo, and if so, whether it is regulated by previously known physiological stimuli of p53, such as DNA damage.	transcription
73489	2	336407	7	NULL	NULL	0	NULL	p53	GP		bind					DNA	NucleicAcid				NULL	in vitro	0	NULL	NULL	NULL	gw60_molcellbiol_19_2_1202_s_169	9891054	Our observations that PCAF specifically acetylates p53 at K320, that this acetylation stimulates p53's DNA binding in vitro, and that alteration of this residue partially lowers p53 transcriptional activity in vivo raised the question of whether the acetylation occurs in vivo, and if so, whether it is regulated by previously known physiological stimuli of p53, such as DNA damage.	transcription
73490	3	336407	7	NULL	NULL	0	NULL	statement 1	Process		stimulate					statement 2	Process				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_2_1202_s_169	9891054	Our observations that PCAF specifically acetylates p53 at K320, that this acetylation stimulates p53's DNA binding in vitro, and that alteration of this residue partially lowers p53 transcriptional activity in vivo raised the question of whether the acetylation occurs in vivo, and if so, whether it is regulated by previously known physiological stimuli of p53, such as DNA damage.	transcription
73491	4	336407	7	NULL	NULL	0	NULL	p53	GP	alteration of	lowers		partially	K320		p53	GP	transcriptional activity of 			NULL	in vivo	0	NULL	NULL	NULL	gw60_molcellbiol_19_2_1202_s_169	9891054	Our observations that PCAF specifically acetylates p53 at K320, that this acetylation stimulates p53's DNA binding in vitro, and that alteration of this residue partially lowers p53 transcriptional activity in vivo raised the question of whether the acetylation occurs in vivo, and if so, whether it is regulated by previously known physiological stimuli of p53, such as DNA damage.	transcription
73492	5	336407	7	NULL	NULL	0	NULL	DNA damage	Process		physiological stimuli of					p53	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_2_1202_s_169	9891054	Our observations that PCAF specifically acetylates p53 at K320, that this acetylation stimulates p53's DNA binding in vitro, and that alteration of this residue partially lowers p53 transcriptional activity in vivo raised the question of whether the acetylation occurs in vivo, and if so, whether it is regulated by previously known physiological stimuli of p53, such as DNA damage.	transcription
73493	1	336408	7	NULL	NULL	NULL	NULL	UV irradiation	PhysicalPhenomenon		induce					p53	GP	cytoplasmic			NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_281_3_1394_s_85	16291740	Importantly, cytoplasmic p53 induced by UV irradiation is acetylated, as it can be recognized by an antibody specific for the acetylated p53 ( Fig. 1 F,  lane 3, upper panel).	transcription
73494	2	336408	7	NULL	NULL	0	NULL	statement 1	Process		acetylate					p53	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_3_1394_s_85	16291740	Importantly, cytoplasmic p53 induced by UV irradiation is acetylated, as it can be recognized by an antibody specific for the acetylated p53 ( Fig. 1 F,  lane 3, upper panel).	transcription
73495	3	336408	7	NULL	NULL	0	NULL	p53 antibody	GP	acetylated	recognize					p53	GP	acetylated			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_281_3_1394_s_85	16291740	Importantly, cytoplasmic p53 induced by UV irradiation is acetylated, as it can be recognized by an antibody specific for the acetylated p53 ( Fig. 1 F,  lane 3, upper panel).	transcription
73496	1	336409	7	NULL	NULL	0	NULL	hGcn5	GP		interacts with		specifically			p53	GP	acetylated			NULL		0	NULL	NULL	NULL	gw60_molcell_8_6_1243_s_239	11779500	hGcn5 also interacted specifically with acetylated p53   (Figure 7A), indicating that TRRAP/hGcn5 complex  (Vassilev et al., 1998  ) binds to acetylated p53.	transcription
73497	2	336409	7	NULL	NULL	0	NULL	TRRAP/hGcn5 complex 	GP		bind					p53	GP	acetylated			NULL		0	NULL	NULL	NULL	gw60_molcell_8_6_1243_s_239	11779500	hGcn5 also interacted specifically with acetylated p53   (Figure 7A), indicating that TRRAP/hGcn5 complex  (Vassilev et al., 1998  ) binds to acetylated p53.	transcription
73498	1	336410	7	NULL	NULL	0	NULL	p300	GP		catalyze					p53	GP	acetylation of	lysine 382 residue		NULL		0	NULL	NULL	NULL	gw70_embo_24_13_2425_s_141	15933712	As expected, the acetylase/coactivator  p300 catalyzed the acetylation of p53 lysine 382 residue ( Figure 5E, lane 2), while coexpressing ATF3, if anything, augmented acetylation ( Figure 5E, lane 3).	transcription
73499	2	336410	7	NULL	NULL	0	NULL	p300	GP		is a type of					acetylase/coactivator	GP				NULL		0	NULL	NULL	NULL	gw70_embo_24_13_2425_s_141	15933712	As expected, the acetylase/coactivator  p300 catalyzed the acetylation of p53 lysine 382 residue ( Figure 5E, lane 2), while coexpressing ATF3, if anything, augmented acetylation ( Figure 5E, lane 3).	transcription
73500	3	336410	7	NULL	NULL	0	NULL	 ATF3	GP		augments					statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_embo_24_13_2425_s_141	15933712	As expected, the acetylase/coactivator  p300 catalyzed the acetylation of p53 lysine 382 residue ( Figure 5E, lane 2), while coexpressing ATF3, if anything, augmented acetylation ( Figure 5E, lane 3).	transcription
73501	1	336411	7	NULL	NULL	0	NULL	Daxx	GP		interacts with					p53	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_50566_s_150	15364927	Because mutation of either PCAF or p300/CBP acetylation sites into alanine is sufficient to inhibit Daxx-p53 interaction, acetylation by either acetylase could potentially block the binding of Daxx to p53.	transcription
73502	2	336411	7	NULL	NULL	0	NULL	PCAF	GP	mutant	inhibit			acetylation site;;alanine		statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_50566_s_150	15364927	Because mutation of either PCAF or p300/CBP acetylation sites into alanine is sufficient to inhibit Daxx-p53 interaction, acetylation by either acetylase could potentially block the binding of Daxx to p53.	transcription
73503	3	336411	7	NULL	NULL	0	NULL	p300/CBP	GP	mutant	inhibit			acetylation site;;alanine		statement 1	Process				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_50566_s_150	15364927	Because mutation of either PCAF or p300/CBP acetylation sites into alanine is sufficient to inhibit Daxx-p53 interaction, acetylation by either acetylase could potentially block the binding of Daxx to p53.	transcription
73504	4	336411	7	NULL	NULL	0	NULL	PCAF	GP		acetylate					p53	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_50566_s_150	15364927	Because mutation of either PCAF or p300/CBP acetylation sites into alanine is sufficient to inhibit Daxx-p53 interaction, acetylation by either acetylase could potentially block the binding of Daxx to p53.	transcription
73505	5	336411	7	NULL	NULL	0	NULL	p300/CBP	GP		acetylate					p53	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_50566_s_150	15364927	Because mutation of either PCAF or p300/CBP acetylation sites into alanine is sufficient to inhibit Daxx-p53 interaction, acetylation by either acetylase could potentially block the binding of Daxx to p53.	transcription
73506	6	336411	7	NULL	NULL	NULL	NULL	statement 4	Process		block		potentially			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_48_50566_s_150	15364927	Because mutation of either PCAF or p300/CBP acetylation sites into alanine is sufficient to inhibit Daxx-p53 interaction, acetylation by either acetylase could potentially block the binding of Daxx to p53.	transcription
73507	7	336411	7	NULL	NULL	NULL	NULL	statement 5	Process		block		potentially			statement 1	Process				NULL		NULL	NULL	NULL	NULL	gw70_jbiolchem_279_48_50566_s_150	15364927	Because mutation of either PCAF or p300/CBP acetylation sites into alanine is sufficient to inhibit Daxx-p53 interaction, acetylation by either acetylase could potentially block the binding of Daxx to p53.	transcription
73508	8	336411	7	NULL	NULL	0	NULL	PCAF	GP		is a type of					acetylase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_50566_s_150	15364927	Because mutation of either PCAF or p300/CBP acetylation sites into alanine is sufficient to inhibit Daxx-p53 interaction, acetylation by either acetylase could potentially block the binding of Daxx to p53.	transcription
73509	9	336411	7	NULL	NULL	0	NULL	p300/CBP	GP		is a type of					acetylase	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_279_48_50566_s_150	15364927	Because mutation of either PCAF or p300/CBP acetylation sites into alanine is sufficient to inhibit Daxx-p53 interaction, acetylation by either acetylase could potentially block the binding of Daxx to p53.	transcription
73510	1	336412	7	NULL	NULL	0	NULL	Mdm2 protein	GP	endogenous	complex with					p300	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3704_s_35	10207094	In cells, most of the endogenous Mdm2 protein is complexed with the histone acetylase p300, and Grossman et al. have shown that the specific interaction between p300 and Mdm2 is required for the degradation of p53 ( 18).	transcription
73511	2	336412	7	NULL	NULL	0	NULL	statement 1	Process		required for					p53	GP	degradation of			NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3704_s_35	10207094	In cells, most of the endogenous Mdm2 protein is complexed with the histone acetylase p300, and Grossman et al. have shown that the specific interaction between p300 and Mdm2 is required for the degradation of p53 ( 18).	transcription
73512	3	336412	7	NULL	NULL	0	NULL	p300	GP		is a type of					histone acetylase	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_19_5_3704_s_35	10207094	In cells, most of the endogenous Mdm2 protein is complexed with the histone acetylase p300, and Grossman et al. have shown that the specific interaction between p300 and Mdm2 is required for the degradation of p53 ( 18).	transcription
73513	1	336413	7	NULL	NULL	0	NULL	p300	GP		acetylate					p53	GP				NULL		0	NULL	NULL	NULL	gw70_pnas_101_5_1273_s_7	14732695	p300 is known to acetylate p53 in response to DNA damage, and when MSI+ cells null for p300 activity are forced to reexpress exogenous  p300 cells show slower growth and a flatter morphology.	transcription
73514	2	336413	7	NULL	NULL	0	NULL	statement 1	Process		in response to					DNA damage	Process				NULL		0	NULL	NULL	NULL	gw70_pnas_101_5_1273_s_7	14732695	p300 is known to acetylate p53 in response to DNA damage, and when MSI+ cells null for p300 activity are forced to reexpress exogenous  p300 cells show slower growth and a flatter morphology.	transcription
73515	1	336414	7	NULL	NULL	0	NULL	CBP 	GP		acetylate					nonhistone proteins	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1404_s_23	11158325	The coactivators CBP and pCAF can also acetylate nonhistone proteins, including transcription factors p53, E2F1, ELKF, GATA 1, TFIIF, and TFIIEbeta and the nuclear receptor coactivator ACTR (reviewed in reference  29).	transcription
73516	2	336414	7	NULL	NULL	0	NULL	pCAF	GP		acetylate					nonhistone proteins	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1404_s_23	11158325	The coactivators CBP and pCAF can also acetylate nonhistone proteins, including transcription factors p53, E2F1, ELKF, GATA 1, TFIIF, and TFIIEbeta and the nuclear receptor coactivator ACTR (reviewed in reference  29).	transcription
73517	3	336414	7	NULL	NULL	0	NULL	CBP	GP		acetylate					p53	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1404_s_23	11158325	The coactivators CBP and pCAF can also acetylate nonhistone proteins, including transcription factors p53, E2F1, ELKF, GATA 1, TFIIF, and TFIIEbeta and the nuclear receptor coactivator ACTR (reviewed in reference  29).	transcription
73518	4	336414	7	NULL	NULL	0	NULL	pCAF	GP		acetylate					p53	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1404_s_23	11158325	The coactivators CBP and pCAF can also acetylate nonhistone proteins, including transcription factors p53, E2F1, ELKF, GATA 1, TFIIF, and TFIIEbeta and the nuclear receptor coactivator ACTR (reviewed in reference  29).	transcription
73519	5	336414	7	NULL	NULL	0	NULL	CBP	GP		acetylate					E2F1	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1404_s_23	11158325	The coactivators CBP and pCAF can also acetylate nonhistone proteins, including transcription factors p53, E2F1, ELKF, GATA 1, TFIIF, and TFIIEbeta and the nuclear receptor coactivator ACTR (reviewed in reference  29).	transcription
73520	6	336414	7	NULL	NULL	0	NULL	pCAF	GP		acetylate					E2F1	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1404_s_23	11158325	The coactivators CBP and pCAF can also acetylate nonhistone proteins, including transcription factors p53, E2F1, ELKF, GATA 1, TFIIF, and TFIIEbeta and the nuclear receptor coactivator ACTR (reviewed in reference  29).	transcription
73521	7	336414	7	NULL	NULL	0	NULL	CBP	GP		acetylate					ELKF	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1404_s_23	11158325	The coactivators CBP and pCAF can also acetylate nonhistone proteins, including transcription factors p53, E2F1, ELKF, GATA 1, TFIIF, and TFIIEbeta and the nuclear receptor coactivator ACTR (reviewed in reference  29).	transcription
73522	8	336414	7	NULL	NULL	0	NULL	pCAF	GP		acetylate					ELKF	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1404_s_23	11158325	The coactivators CBP and pCAF can also acetylate nonhistone proteins, including transcription factors p53, E2F1, ELKF, GATA 1, TFIIF, and TFIIEbeta and the nuclear receptor coactivator ACTR (reviewed in reference  29).	transcription
73523	9	336414	7	NULL	NULL	0	NULL	CBP	GP		acetylate					GATA 1	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1404_s_23	11158325	The coactivators CBP and pCAF can also acetylate nonhistone proteins, including transcription factors p53, E2F1, ELKF, GATA 1, TFIIF, and TFIIEbeta and the nuclear receptor coactivator ACTR (reviewed in reference  29).	transcription
73524	10	336414	7	NULL	NULL	0	NULL	pCAF	GP		acetylate					GATA 1	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1404_s_23	11158325	The coactivators CBP and pCAF can also acetylate nonhistone proteins, including transcription factors p53, E2F1, ELKF, GATA 1, TFIIF, and TFIIEbeta and the nuclear receptor coactivator ACTR (reviewed in reference  29).	transcription
73525	11	336414	7	NULL	NULL	0	NULL	CBP	GP		acetylate					TFIIF	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1404_s_23	11158325	The coactivators CBP and pCAF can also acetylate nonhistone proteins, including transcription factors p53, E2F1, ELKF, GATA 1, TFIIF, and TFIIEbeta and the nuclear receptor coactivator ACTR (reviewed in reference  29).	transcription
73526	12	336414	7	NULL	NULL	0	NULL	pCAF	GP		acetylate					TFIIF	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1404_s_23	11158325	The coactivators CBP and pCAF can also acetylate nonhistone proteins, including transcription factors p53, E2F1, ELKF, GATA 1, TFIIF, and TFIIEbeta and the nuclear receptor coactivator ACTR (reviewed in reference  29).	transcription
73527	13	336414	7	NULL	NULL	0	NULL	CBP	GP		acetylate					TFIIEbeta	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1404_s_23	11158325	The coactivators CBP and pCAF can also acetylate nonhistone proteins, including transcription factors p53, E2F1, ELKF, GATA 1, TFIIF, and TFIIEbeta and the nuclear receptor coactivator ACTR (reviewed in reference  29).	transcription
73528	14	336414	7	NULL	NULL	0	NULL	pCAF	GP		acetylate					TFIIEbeta	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1404_s_23	11158325	The coactivators CBP and pCAF can also acetylate nonhistone proteins, including transcription factors p53, E2F1, ELKF, GATA 1, TFIIF, and TFIIEbeta and the nuclear receptor coactivator ACTR (reviewed in reference  29).	transcription
73529	15	336414	7	NULL	NULL	0	NULL	CBP	GP		acetylate					ACTR	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1404_s_23	11158325	The coactivators CBP and pCAF can also acetylate nonhistone proteins, including transcription factors p53, E2F1, ELKF, GATA 1, TFIIF, and TFIIEbeta and the nuclear receptor coactivator ACTR (reviewed in reference  29).	transcription
73530	16	336414	7	NULL	NULL	0	NULL	pCAF	GP		acetylate					ACTR	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1404_s_23	11158325	The coactivators CBP and pCAF can also acetylate nonhistone proteins, including transcription factors p53, E2F1, ELKF, GATA 1, TFIIF, and TFIIEbeta and the nuclear receptor coactivator ACTR (reviewed in reference  29).	transcription
73531	17	336414	7	NULL	NULL	0	NULL	CBP	GP		is a type of					coactivator	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1404_s_23	11158325	The coactivators CBP and pCAF can also acetylate nonhistone proteins, including transcription factors p53, E2F1, ELKF, GATA 1, TFIIF, and TFIIEbeta and the nuclear receptor coactivator ACTR (reviewed in reference  29).	transcription
73532	18	336414	7	NULL	NULL	0	NULL	pCAF	GP		is a type of					coactivator	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1404_s_23	11158325	The coactivators CBP and pCAF can also acetylate nonhistone proteins, including transcription factors p53, E2F1, ELKF, GATA 1, TFIIF, and TFIIEbeta and the nuclear receptor coactivator ACTR (reviewed in reference  29).	transcription
73533	19	336414	7	NULL	NULL	0	NULL	p53	GP		is a type of					transcription factor	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1404_s_23	11158325	The coactivators CBP and pCAF can also acetylate nonhistone proteins, including transcription factors p53, E2F1, ELKF, GATA 1, TFIIF, and TFIIEbeta and the nuclear receptor coactivator ACTR (reviewed in reference  29).	transcription
73534	20	336414	7	NULL	NULL	0	NULL	 E2F1	GP		is a type of					transcription factor	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1404_s_23	11158325	The coactivators CBP and pCAF can also acetylate nonhistone proteins, including transcription factors p53, E2F1, ELKF, GATA 1, TFIIF, and TFIIEbeta and the nuclear receptor coactivator ACTR (reviewed in reference  29).	transcription
73535	21	336414	7	NULL	NULL	0	NULL	GATA 1	GP		is a type of					transcription factor	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1404_s_23	11158325	The coactivators CBP and pCAF can also acetylate nonhistone proteins, including transcription factors p53, E2F1, ELKF, GATA 1, TFIIF, and TFIIEbeta and the nuclear receptor coactivator ACTR (reviewed in reference  29).	transcription
73536	22	336414	7	NULL	NULL	0	NULL	TFIIF	GP		is a type of					transcription factor	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1404_s_23	11158325	The coactivators CBP and pCAF can also acetylate nonhistone proteins, including transcription factors p53, E2F1, ELKF, GATA 1, TFIIF, and TFIIEbeta and the nuclear receptor coactivator ACTR (reviewed in reference  29).	transcription
73537	23	336414	7	NULL	NULL	0	NULL	TFIIEbeta	GP		is a type of					transcription factor	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1404_s_23	11158325	The coactivators CBP and pCAF can also acetylate nonhistone proteins, including transcription factors p53, E2F1, ELKF, GATA 1, TFIIF, and TFIIEbeta and the nuclear receptor coactivator ACTR (reviewed in reference  29).	transcription
73538	24	336414	7	NULL	NULL	0	NULL	ACTR	GP		is a type of					nuclear receptor coactivator 	GP				NULL		0	NULL	NULL	NULL	gw60_molcellbiol_21_4_1404_s_23	11158325	The coactivators CBP and pCAF can also acetylate nonhistone proteins, including transcription factors p53, E2F1, ELKF, GATA 1, TFIIF, and TFIIEbeta and the nuclear receptor coactivator ACTR (reviewed in reference  29).	transcription
73539	1	336415	7	NULL	NULL	0	NULL	p300/CBP	GP		acetylate					p53	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_48_34020_s_47	10567368	p300/CBP have also been shown to acetylate several transcription factors including p53 ( 69), NF-Y ( 70), and GATA-1 ( 71), which influences their binding to DNA.	transcription
73540	2	336415	7	NULL	NULL	0	NULL	p300/CBP	GP		acetylate					NF-Y 	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_48_34020_s_47	10567368	p300/CBP have also been shown to acetylate several transcription factors including p53 ( 69), NF-Y ( 70), and GATA-1 ( 71), which influences their binding to DNA.	transcription
73541	3	336415	7	NULL	NULL	0	NULL	p300/CBP	GP		acetylate					GATA-1	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_48_34020_s_47	10567368	p300/CBP have also been shown to acetylate several transcription factors including p53 ( 69), NF-Y ( 70), and GATA-1 ( 71), which influences their binding to DNA.	transcription
73542	4	336415	7	NULL	NULL	0	NULL	p53	GP		bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_48_34020_s_47	10567368	p300/CBP have also been shown to acetylate several transcription factors including p53 ( 69), NF-Y ( 70), and GATA-1 ( 71), which influences their binding to DNA.	transcription
73543	5	336415	7	NULL	NULL	0	NULL	NF-Y 	GP		bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_48_34020_s_47	10567368	p300/CBP have also been shown to acetylate several transcription factors including p53 ( 69), NF-Y ( 70), and GATA-1 ( 71), which influences their binding to DNA.	transcription
73544	6	336415	7	NULL	NULL	0	NULL	GATA-1	GP		bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_48_34020_s_47	10567368	p300/CBP have also been shown to acetylate several transcription factors including p53 ( 69), NF-Y ( 70), and GATA-1 ( 71), which influences their binding to DNA.	transcription
73545	7	336415	7	NULL	NULL	0	NULL	statement 1	Process		influence					statement 4	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_48_34020_s_47	10567368	p300/CBP have also been shown to acetylate several transcription factors including p53 ( 69), NF-Y ( 70), and GATA-1 ( 71), which influences their binding to DNA.	transcription
73546	8	336415	7	NULL	NULL	0	NULL	statement 2	Process		influence					statement 5	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_48_34020_s_47	10567368	p300/CBP have also been shown to acetylate several transcription factors including p53 ( 69), NF-Y ( 70), and GATA-1 ( 71), which influences their binding to DNA.	transcription
73547	9	336415	7	NULL	NULL	0	NULL	statement 3	Process		influence					statement 6	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_48_34020_s_47	10567368	p300/CBP have also been shown to acetylate several transcription factors including p53 ( 69), NF-Y ( 70), and GATA-1 ( 71), which influences their binding to DNA.	transcription
73548	10	336415	7	NULL	NULL	0	NULL	p53	GP		is a type of					transcription factor	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_48_34020_s_47	10567368	p300/CBP have also been shown to acetylate several transcription factors including p53 ( 69), NF-Y ( 70), and GATA-1 ( 71), which influences their binding to DNA.	transcription
73549	11	336415	7	NULL	NULL	0	NULL	 NF-Y	GP		is a type of					transcription factor	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_48_34020_s_47	10567368	p300/CBP have also been shown to acetylate several transcription factors including p53 ( 69), NF-Y ( 70), and GATA-1 ( 71), which influences their binding to DNA.	transcription
73550	12	336415	7	NULL	NULL	0	NULL	GATA-1	GP		is a type of					transcription factor	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_274_48_34020_s_47	10567368	p300/CBP have also been shown to acetylate several transcription factors including p53 ( 69), NF-Y ( 70), and GATA-1 ( 71), which influences their binding to DNA.	transcription
73551	1	336416	7	NULL	NULL	0	NULL	HDAC1	GP		deacetylate					histones	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_39_37439_s_383	12876282	In addition to deacetylating histones, HDAC1,-2, and-3 are able to deacetylate p53 at the C terminus that can be acetylated by p300/CBP  in vivo ( ,  ), resulting in suppression of the p53 transactivation activity.	transcription
73552	2	336416	7	NULL	NULL	0	NULL	HDAC2	GP		deacetylate					histones	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_39_37439_s_383	12876282	In addition to deacetylating histones, HDAC1,-2, and-3 are able to deacetylate p53 at the C terminus that can be acetylated by p300/CBP  in vivo ( ,  ), resulting in suppression of the p53 transactivation activity.	transcription
73553	3	336416	7	NULL	NULL	0	NULL	HDAC3	GP		deacetylate					histones	GP				NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_39_37439_s_383	12876282	In addition to deacetylating histones, HDAC1,-2, and-3 are able to deacetylate p53 at the C terminus that can be acetylated by p300/CBP  in vivo ( ,  ), resulting in suppression of the p53 transactivation activity.	transcription
73554	4	336416	7	NULL	NULL	0	NULL	HDAC1	GP		deacetylate					p53	GP		C terminus		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_39_37439_s_383	12876282	In addition to deacetylating histones, HDAC1,-2, and-3 are able to deacetylate p53 at the C terminus that can be acetylated by p300/CBP  in vivo ( ,  ), resulting in suppression of the p53 transactivation activity.	transcription
73555	5	336416	7	NULL	NULL	0	NULL	HDAC2	GP		deacetylate					p53	GP		C terminus		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_39_37439_s_383	12876282	In addition to deacetylating histones, HDAC1,-2, and-3 are able to deacetylate p53 at the C terminus that can be acetylated by p300/CBP  in vivo ( ,  ), resulting in suppression of the p53 transactivation activity.	transcription
73556	6	336416	7	NULL	NULL	0	NULL	HDAC3	GP		deacetylate					p53	GP		C terminus		NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_39_37439_s_383	12876282	In addition to deacetylating histones, HDAC1,-2, and-3 are able to deacetylate p53 at the C terminus that can be acetylated by p300/CBP  in vivo ( ,  ), resulting in suppression of the p53 transactivation activity.	transcription
73557	7	336416	7	NULL	NULL	0	NULL	p300/CBP	GP		acetylate					p53	GP				NULL	in vivo	0	NULL	NULL	NULL	gw70_jbiolchem_278_39_37439_s_383	12876282	In addition to deacetylating histones, HDAC1,-2, and-3 are able to deacetylate p53 at the C terminus that can be acetylated by p300/CBP  in vivo ( ,  ), resulting in suppression of the p53 transactivation activity.	transcription
73558	8	336416	7	NULL	NULL	0	NULL	statement 4	Process		suppress					p53	GP	transactivation activity of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_39_37439_s_383	12876282	In addition to deacetylating histones, HDAC1,-2, and-3 are able to deacetylate p53 at the C terminus that can be acetylated by p300/CBP  in vivo ( ,  ), resulting in suppression of the p53 transactivation activity.	transcription
73559	9	336416	7	NULL	NULL	0	NULL	statement 5	Process		suppress					p53	GP	transactivation activity of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_39_37439_s_383	12876282	In addition to deacetylating histones, HDAC1,-2, and-3 are able to deacetylate p53 at the C terminus that can be acetylated by p300/CBP  in vivo ( ,  ), resulting in suppression of the p53 transactivation activity.	transcription
73560	10	336416	7	NULL	NULL	0	NULL	statement 6	Process		suppress					p53	GP	transactivation activity of			NULL		0	NULL	NULL	NULL	gw70_jbiolchem_278_39_37439_s_383	12876282	In addition to deacetylating histones, HDAC1,-2, and-3 are able to deacetylate p53 at the C terminus that can be acetylated by p300/CBP  in vivo ( ,  ), resulting in suppression of the p53 transactivation activity.	transcription
73561	1	336417	7	NULL	NULL	NULL	NULL	TSA	Chemical		inhibit		effectively			p53 deacetylase	GP				NULL	A549 cells	NULL	NULL	NULL	NULL	gw60_embo_20_6_1331_s_187	11250899	As shown in Figure  6A (top panel), TSA treatment effectively inhibited the p53 deacetylase and increased the levels of acetylated p53 in A549 cells.	transcription
73562	2	336417	7	NULL	NULL	0	NULL	statement 1	Process		increase					p53	GP	acetylated			NULL	A549 cells	0	NULL	NULL	NULL	gw60_embo_20_6_1331_s_187	11250899	As shown in Figure  6A (top panel), TSA treatment effectively inhibited the p53 deacetylase and increased the levels of acetylated p53 in A549 cells.	transcription
73563	1	336418	7	NULL	NULL	NULL	NULL	CBP/p300	GP		mediate					p53	GP	acetylation of			NULL	in vivo	NULL	NULL	NULL	NULL	gw60_cell_107_2_137_s_17	11672522	By developing site-specific acetylated p53  antibodies, CBP/p300 mediated acetylation of p53 was further  confirmed in vivo by a number of  studies (reviewed in Appella and Anderson, 2000   ).	transcription
73564	1	336419	7	NULL	NULL	0	NULL	p53	GP	mutant	acteylated by			lysine residue		p300	GP				NULL		0	NULL	NULL	NULL	gw60_molcell_8_1_57_s_273	11511360	We find that p53 proteins containing mutations in lysine residues acetylated by p300 are as active as wild-type p53 in regulating p21 transcription in vitro.	transcription
73565	2	336419	7	NULL	NULL	0	NULL	p53	GP	wild-type	regulate					p21	GP	transcription of			NULL	in vitro	0	NULL	NULL	NULL	gw60_molcell_8_1_57_s_273	11511360	We find that p53 proteins containing mutations in lysine residues acetylated by p300 are as active as wild-type p53 in regulating p21 transcription in vitro.	transcription
73566	3	336419	7	NULL	NULL	0	NULL	p53	GP	mutant	regulate			lysine residue		p21	GP	transcription of			NULL	in vitro	0	NULL	NULL	NULL	gw60_molcell_8_1_57_s_273	11511360	We find that p53 proteins containing mutations in lysine residues acetylated by p300 are as active as wild-type p53 in regulating p21 transcription in vitro.	transcription
73567	4	336419	7	NULL	NULL	0	NULL	statement 2	Process		is as active as					statement 3	Process				NULL		0	NULL	NULL	NULL	gw60_molcell_8_1_57_s_273	11511360	We find that p53 proteins containing mutations in lysine residues acetylated by p300 are as active as wild-type p53 in regulating p21 transcription in vitro.	transcription
73568	1	336420	7	NULL	NULL	0	NULL	PCAF	GP		acetylate					p53	GP		lysine		NULL	in vitro	0	NULL	NULL	NULL	gw60_molcellbiol_19_2_1202_s_204	9891054	In particular, under in vivo conditions that cause DNA damage, which potentiate p53 activity, increased p53 acetylation is detected at lysines acetylated in vitro by PCAF and p300.	transcription
73569	2	336420	7	NULL	NULL	0	NULL	p300	GP		acetylate					p53	GP		lysine		NULL	in vitro	0	NULL	NULL	NULL	gw60_molcellbiol_19_2_1202_s_204	9891054	In particular, under in vivo conditions that cause DNA damage, which potentiate p53 activity, increased p53 acetylation is detected at lysines acetylated in vitro by PCAF and p300.	transcription
73570	1	336421	7	NULL	NULL	0	NULL	HDAC	GP		down-regulates					p53	GP	activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20436_s_5	10777477	Down-regulation of p53 activity by HDACs is HDAC dosage-dependent, requires the deacetylase activity of HDACs, and depends on the region of p53 that is acetylated by p300/CREB-binding protein (CBP).	transcription
73571	2	336421	7	NULL	NULL	0	NULL	statement 1	Process		depends on					HDAC	GP	dose of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20436_s_5	10777477	Down-regulation of p53 activity by HDACs is HDAC dosage-dependent, requires the deacetylase activity of HDACs, and depends on the region of p53 that is acetylated by p300/CREB-binding protein (CBP).	transcription
73572	3	336421	7	NULL	NULL	0	NULL	statement 1	Process		requires					HDAC	GP	deacetylase activity of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20436_s_5	10777477	Down-regulation of p53 activity by HDACs is HDAC dosage-dependent, requires the deacetylase activity of HDACs, and depends on the region of p53 that is acetylated by p300/CREB-binding protein (CBP).	transcription
73573	4	336421	7	NULL	NULL	0	NULL	p300/CREB-binding protein 	GP		acetylate					p53	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20436_s_5	10777477	Down-regulation of p53 activity by HDACs is HDAC dosage-dependent, requires the deacetylase activity of HDACs, and depends on the region of p53 that is acetylated by p300/CREB-binding protein (CBP).	transcription
73574	5	336421	7	NULL	NULL	0	NULL	statement 1	Process		depends on					p53	GP	acetylated region of			NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20436_s_5	10777477	Down-regulation of p53 activity by HDACs is HDAC dosage-dependent, requires the deacetylase activity of HDACs, and depends on the region of p53 that is acetylated by p300/CREB-binding protein (CBP).	transcription
73575	6	336421	7	NULL	NULL	0	NULL	CBP	GP		is					CREB-binding protein	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_27_20436_s_5	10777477	Down-regulation of p53 activity by HDACs is HDAC dosage-dependent, requires the deacetylase activity of HDACs, and depends on the region of p53 that is acetylated by p300/CREB-binding protein (CBP).	transcription
73576	1	336422	7	NULL	NULL	0	NULL	p53	GP	acetylation of	depends on					DNA damage	Process				NULL	cultured cells	0	NULL	NULL	NULL	gw60_jbiolchem_275_29_21953_s_251	10777508	As p53 is acetylated in a DNA damage-dependent manner in cultured cells ( 6), the binding mode of PCAF to p53 might be regulated via a signaling network.	transcription
73577	2	336422	7	NULL	NULL	0	NULL	PCAF	GP		bind					p53	GP				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_29_21953_s_251	10777508	As p53 is acetylated in a DNA damage-dependent manner in cultured cells ( 6), the binding mode of PCAF to p53 might be regulated via a signaling network.	transcription
73578	3	336422	7	NULL	NULL	0	NULL	statement 2	Process		regulated via					signaling network	Process				NULL		0	NULL	NULL	NULL	gw60_jbiolchem_275_29_21953_s_251	10777508	As p53 is acetylated in a DNA damage-dependent manner in cultured cells ( 6), the binding mode of PCAF to p53 might be regulated via a signaling network.	transcription
67794	1	346003	9	NULL	NULL	NULL	NULL	deletion experiments	ResearchActivity		identified					heat regulation regions	GP				NULL	several different heat shock genes	NULL	NULL	NULL	NULL	tag10_molcellbiol_8_9_3761_s_2	3146692	 Regions responsible for heat regulation have been identified previously by deletion experiments with several different heat shock genes .	tag10-1
67801	1	346007	9	NULL	NULL	NULL	NULL	nucleotides at two positions	NucleicAcid		upstream					GAA segments	NucleicAcid				NULL		NULL	NULL	NULL	NULL	tag10_molcellbiol_8_9_3761_s_6	3146692	 Second , the nucleotides at the two positions immediately upstream from GAA segments played an important role in defining the competence of regulatory elements .	tag10-1
67802	2	346007	9	NULL	NULL	NULL	NULL	statement 1	NucleicAcid		plays a role in					heat shock regulatory elements	NucleicAcid	competence of			NULL		NULL	NULL	NULL	NULL	tag10_molcellbiol_8_9_3761_s_6	3146692	 Second , the nucleotides at the two positions immediately upstream from GAA segments played an important role in defining the competence of regulatory elements .	tag10-1
67900	1	346010	9	NULL	NULL	0	NULL	hsp70 genes	GP		expression by					heat-regulation	ResearchActivity				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_8_9_3761_s_9	3146692	 In most cell types , the genes were expressed in a heat-regulated fashion .	tag10-1
67909	1	346013	9	NULL	NULL	0	NULL	CNNGAANNTTCNNG	NucleicAcid		is					heat shock consensus sequence	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_8_9_3761_s_12	3146692	 Comparison of the -45 to -65 sequence of Drosophila hsp70 genes and of analogous sequences in other hsp genes led to the establishment of a heat shock consensus sequence , CNNGAANNTTCNNG ,  ( 31  ) , where N is any nucleotide .	tag10-1
67910	2	346013	9	NULL	NULL	0	NULL	heat shock consensus sequence	NucleicAcid		analogous to					hsp genes	GP	other			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_8_9_3761_s_12	3146692	 Comparison of the -45 to -65 sequence of Drosophila hsp70 genes and of analogous sequences in other hsp genes led to the establishment of a heat shock consensus sequence , CNNGAANNTTCNNG ,  ( 31  ) , where N is any nucleotide .	tag10-1
67911	1	346014	9	NULL	NULL	0	NULL	Heat Shock Factors			cause					hsp genes		Transcriptional activation of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_8_9_3761_s_13	3146692	 Factors binding to this type of sequence have been identified  ( 17 , 28 , 37 , 45 , 47 , 48  ) , and two groups have purified such factors from Drosophila nuclear extracts and have shown that they are specifically involved in transcriptional activation of hsp genes ( 28 , 45 , 48  ) .	tag10-1
67912	1	346015	9	NULL	NULL	0	NULL	heat shock transcription elements	Process		important for					heat shock regulation	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_8_9_3761_s_14	3146692	 Since the sequences described above are the only elements specifically required for heat regulation and are also binding sites for hsp gene-specific transcription factors , they are of central importance for the understanding of heat shock regulation .	tag10-1
67915	1	346019	9	NULL	NULL	NULL	NULL	Plasmids	NucleicAcid		derived from					D88 contruct	NucleicAcid				NULL		NULL	NULL	NULL	NULL	tag10_molcellbiol_8_9_3761_s_18	3146692	 Plasmids  ( Fig . 1 and 2  ) were derived from constructs D88 and D50  ( 2  ) .	tag10-1
67916	2	346019	9	NULL	NULL	0	NULL	Plasmids	NucleicAcid		derived from					D50 contruct	NucleicAcid				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_8_9_3761_s_18	3146692	 Plasmids  ( Fig . 1 and 2  ) were derived from constructs D88 and D50  ( 2  ) .	tag10-1
67934	1	346024	9	NULL	NULL	0	NULL	Synthetic linkers	NucleicAcid		obtained from					New England Biolabs	Facility				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_8_9_3761_s_23	3146692	 Synthetic linkers ( XhoI , BamHI , EcoRI , and SmaI  ) were obtained from New England Biolabs or International Biochemical Co.	tag10-1
67935	2	346024	9	NULL	NULL	0	NULL	Synthetic linkers	NucleicAcid		obtained from					International Biochemical Co	Facility				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_8_9_3761_s_23	3146692	 Synthetic linkers ( XhoI , BamHI , EcoRI , and SmaI  ) were obtained from New England Biolabs or International Biochemical Co.	tag10-1
67936	3	346024	9	NULL	NULL	0	NULL	XhoI	NucleicAcid		is a type of					Synthetic linkers	NucleicAcid				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_8_9_3761_s_23	3146692	 Synthetic linkers ( XhoI , BamHI , EcoRI , and SmaI  ) were obtained from New England Biolabs or International Biochemical Co.	tag10-1
67937	4	346024	9	NULL	NULL	0	NULL	BamHI	NucleicAcid		is a type of					Synthetic linkers	NucleicAcid				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_8_9_3761_s_23	3146692	 Synthetic linkers ( XhoI , BamHI , EcoRI , and SmaI  ) were obtained from New England Biolabs or International Biochemical Co.	tag10-1
67938	5	346024	9	NULL	NULL	0	NULL	EcoRI 	NucleicAcid		is a type of					Synthetic linkers	NucleicAcid				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_8_9_3761_s_23	3146692	 Synthetic linkers ( XhoI , BamHI , EcoRI , and SmaI  ) were obtained from New England Biolabs or International Biochemical Co.	tag10-1
67939	5	346024	9	NULL	NULL	0	NULL	EcoRI 	NucleicAcid		is a type of					Synthetic linkers	NucleicAcid				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_8_9_3761_s_23	3146692	 Synthetic linkers ( XhoI , BamHI , EcoRI , and SmaI  ) were obtained from New England Biolabs or International Biochemical Co.	tag10-1
67940	6	346024	9	NULL	NULL	0	NULL	SmaI	NucleicAcid		is a type of					Synthetic linkers	NucleicAcid				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_8_9_3761_s_23	3146692	 Synthetic linkers ( XhoI , BamHI , EcoRI , and SmaI  ) were obtained from New England Biolabs or International Biochemical Co.	tag10-1
67941	1	346026	9	NULL	NULL	0	NULL	Complementary segments	NucleicAcid		treated with					T4 polynucleotide kinase	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_8_9_3761_s_25	3146692	 Complementary segments were annealed and treated with T4 polynucleotide kinase .	tag10-1
67942	1	346027	9	NULL	NULL	0	NULL	BssHII-Xba I fragment	NucleicAcid		isolated from					clone 122	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_8_9_3761_s_26	3146692	 To prepare XBA8 , a BssHII-Xba I fragment  ( hsp70 sequences from -67 to -244  ) was isolated from clone 122  ( 12  ) , blunted , and inserted into the unique XhoI site ( filled  ) of D50 .	tag10-1
67943	2	346027	9	NULL	NULL	NULL	NULL	BssHII-Xba I fragment	NucleicAcid		inserted into					XhoI site	NucleicAcid	unique			NULL		NULL	NULL	NULL	NULL	tag10_molcellbiol_8_9_3761_s_26	3146692	 To prepare XBA8 , a BssHII-Xba I fragment  ( hsp70 sequences from -67 to -244  ) was isolated from clone 122  ( 12  ) , blunted , and inserted into the unique XhoI site ( filled  ) of D50 .	tag10-1
67944	3	346027	9	NULL	NULL	0	NULL	BssHII-Xba I fragment	NucleicAcid		undergo					Blunting	ResearchActivity				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_8_9_3761_s_26	3146692	 To prepare XBA8 , a BssHII-Xba I fragment  ( hsp70 sequences from -67 to -244  ) was isolated from clone 122  ( 12  ) , blunted , and inserted into the unique XhoI site ( filled  ) of D50 .	tag10-1
67945	4	346027	9	NULL	NULL	0	NULL	Statement 1	ResearchActivity		prepare					XBA8	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_8_9_3761_s_26	3146692	 To prepare XBA8 , a BssHII-Xba I fragment  ( hsp70 sequences from -67 to -244  ) was isolated from clone 122  ( 12  ) , blunted , and inserted into the unique XhoI site ( filled  ) of D50 .	tag10-1
67946	5	346027	9	NULL	NULL	0	NULL	Statement 2	ResearchActivity		prepare					XBA8	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_8_9_3761_s_26	3146692	 To prepare XBA8 , a BssHII-Xba I fragment  ( hsp70 sequences from -67 to -244  ) was isolated from clone 122  ( 12  ) , blunted , and inserted into the unique XhoI site ( filled  ) of D50 .	tag10-1
67963	1	346032	9	NULL	NULL	0	NULL	Sequencing	ResearchActivity		performed by					chemical procedure	ResearchActivity				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_8_9_3761_s_31	3146692	 Sequencing was performed by either the chemical procedure  ( 21  ) or the dideoxy method ( 35  ) .	tag10-1
67964	2	346032	9	NULL	NULL	0	NULL	Sequencing	ResearchActivity		performed by					dideoxy method	ResearchActivity				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_8_9_3761_s_31	3146692	 Sequencing was performed by either the chemical procedure  ( 21  ) or the dideoxy method ( 35  ) .	tag10-1
61278	1	346226	5	NULL	NULL	0	NULL	heat shock factor	GP		interacts with					hsp7O	GP				NULL	in vivo	NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_1	7935376	Interaction between Heat Shock Factor and hsp7O Is Insufficient To Suppress Induction of DNA-Binding Activity In Vivo  The intracellular level of free heat shock proteins, in particular the 70-kDa stress protein family, has been suggested to be the basis of an autoregulatory mechanism by which the cell measures the level of thermal stress and regulates the synthesis of heat shock proteins.	tag10-2
61281	3	346226	5	NULL	NULL	0	NULL	hsp7O	GP		is a member of					stress protein family	GP				NULL		NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_1	7935376	Interaction between Heat Shock Factor and hsp7O Is Insufficient To Suppress Induction of DNA-Binding Activity In Vivo  The intracellular level of free heat shock proteins, in particular the 70-kDa stress protein family, has been suggested to be the basis of an autoregulatory mechanism by which the cell measures the level of thermal stress and regulates the synthesis of heat shock proteins.	tag10-2
61282	4	346226	5	NULL	NULL	0	NULL	hsp7O	GP	intracellular level of;;free	plays a role in					autoregulatory mechanism	Process				NULL		NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_1	7935376	Interaction between Heat Shock Factor and hsp7O Is Insufficient To Suppress Induction of DNA-Binding Activity In Vivo  The intracellular level of free heat shock proteins, in particular the 70-kDa stress protein family, has been suggested to be the basis of an autoregulatory mechanism by which the cell measures the level of thermal stress and regulates the synthesis of heat shock proteins.	tag10-2
61283	5	346226	5	NULL	NULL	0	NULL	cell	Cell		measures					thermal stress	Process	level of			NULL		NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_1	7935376	Interaction between Heat Shock Factor and hsp7O Is Insufficient To Suppress Induction of DNA-Binding Activity In Vivo  The intracellular level of free heat shock proteins, in particular the 70-kDa stress protein family, has been suggested to be the basis of an autoregulatory mechanism by which the cell measures the level of thermal stress and regulates the synthesis of heat shock proteins.	tag10-2
61284	6	346226	5	NULL	NULL	0	NULL	cell	Cell		regulates					heat shock proteins	GP	synthesis of			NULL		NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_1	7935376	Interaction between Heat Shock Factor and hsp7O Is Insufficient To Suppress Induction of DNA-Binding Activity In Vivo  The intracellular level of free heat shock proteins, in particular the 70-kDa stress protein family, has been suggested to be the basis of an autoregulatory mechanism by which the cell measures the level of thermal stress and regulates the synthesis of heat shock proteins.	tag10-2
61285	7	346226	5	NULL	NULL	0	NULL	statement 5	Process		followed by					statement 6	Process				NULL		NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_1	7935376	Interaction between Heat Shock Factor and hsp7O Is Insufficient To Suppress Induction of DNA-Binding Activity In Vivo  The intracellular level of free heat shock proteins, in particular the 70-kDa stress protein family, has been suggested to be the basis of an autoregulatory mechanism by which the cell measures the level of thermal stress and regulates the synthesis of heat shock proteins.	tag10-2
61286	1	346227	5	NULL	NULL	0	NULL	HSF	GP		is					heat shock transcription factor	GP				NULL		NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_2	7935376	It has been proposed that the DNA-binding and oligomeric state of the heat shock transcription factor (HSF) is a principal step in the induction pathway that is responsive to the level of 70-kDa stress protein.	tag10-2
61287	2	346227	5	NULL	NULL	0	NULL	HSF	GP		bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_2	7935376	It has been proposed that the DNA-binding and oligomeric state of the heat shock transcription factor (HSF) is a principal step in the induction pathway that is responsive to the level of 70-kDa stress protein.	tag10-2
61288	3	346227	5	NULL	NULL	0	NULL	induction pathway	Process		is responsive to					70-kDa stress protein	GP	level of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_2	7935376	It has been proposed that the DNA-binding and oligomeric state of the heat shock transcription factor (HSF) is a principal step in the induction pathway that is responsive to the level of 70-kDa stress protein.	tag10-2
61289	4	346227	5	NULL	NULL	0	NULL	statement 2	Process		is a principal step in					statement 3	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_2	7935376	It has been proposed that the DNA-binding and oligomeric state of the heat shock transcription factor (HSF) is a principal step in the induction pathway that is responsive to the level of 70-kDa stress protein.	tag10-2
61290	5	346227	5	NULL	NULL	0	NULL	HSF	GP	oligomeric state of	is a principal step in					statement 3	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_2	7935376	It has been proposed that the DNA-binding and oligomeric state of the heat shock transcription factor (HSF) is a principal step in the induction pathway that is responsive to the level of 70-kDa stress protein.	tag10-2
61291	1	346228	5	NULL	NULL	0	NULL	HSF	GP		is associated with		potentially			70-kDa stress protein	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_3	7935376	To test this hypothesis, we investigated the association between HSF and 70-kDa stress protein by means of a coimmunoprecipitation assay.	tag10-2
61292	1	346229	5	NULL	NULL	0	NULL	70-kDa stress proteins	GP		associate with					HSF	GP	latent			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_4	7935376	We found that 70-kDa stress proteins associate to similar extents with both latent and active fonns of HSF, although unlike other 70-kDa stress protein substrates, the association with HSF was not significantly disrupted in the presence of ATP.	tag10-2
61293	2	346229	5	NULL	NULL	0	NULL	70-kDa stress proteins	GP		associate with					HSF	GP	active			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_4	7935376	We found that 70-kDa stress proteins associate to similar extents with both latent and active fonns of HSF, although unlike other 70-kDa stress protein substrates, the association with HSF was not significantly disrupted in the presence of ATP.	tag10-2
61294	3	346229	5	NULL	NULL	0	NULL	statement 1	Process	affinity of	is similar to					statement 2	Process	affinity of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_4	7935376	We found that 70-kDa stress proteins associate to similar extents with both latent and active fonns of HSF, although unlike other 70-kDa stress protein substrates, the association with HSF was not significantly disrupted in the presence of ATP.	tag10-2
61295	4	346229	5	NULL	NULL	0	NULL	statement 1	Process		is not disrupted by		significantly			ATP	Chemical	presence of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_4	7935376	We found that 70-kDa stress proteins associate to similar extents with both latent and active fonns of HSF, although unlike other 70-kDa stress protein substrates, the association with HSF was not significantly disrupted in the presence of ATP.	tag10-2
61296	5	346229	5	NULL	NULL	0	NULL	statement 2	Process		is not disrupted by					ATP	Chemical	presence of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_4	7935376	We found that 70-kDa stress proteins associate to similar extents with both latent and active fonns of HSF, although unlike other 70-kDa stress protein substrates, the association with HSF was not significantly disrupted in the presence of ATP.	tag10-2
61297	1	346230	5	NULL	NULL	0	NULL	HSF trimer	GP	bacterially purified;;active	is not deactivated with		substantially			70-kDa stress protein	GP	purified			NULL	in vitro	NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_5	7935376	Gel mobility shift assays indicated that active HSF trimers purified from a bacterial expression system could not be substantially deactivated in vitro with purified 70-kDa stress protein and ATP.	tag10-2
61298	2	346230	5	NULL	NULL	0	NULL	HSF trimer	GP	bacterially purified;;active	is not deactivated with		substantially			ATP	Chemical				NULL	in vitro	NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_5	7935376	Gel mobility shift assays indicated that active HSF trimers purified from a bacterial expression system could not be substantially deactivated in vitro with purified 70-kDa stress protein and ATP.	tag10-2
61299	1	346231	5	NULL	NULL	0	NULL	HSF	GP		activates					DNA	NucleicAcid	binding of			NULL	cultured rat cells	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_6	7935376	In addition, elevated concentrations of hsp7O alone could not significantly inhibit induction of the DNA-binding activity of endogenous HSF in cultured rat cells, and the induction was also not inhibited in cultured rat cells or Drosophila cells containing elevated levels of all members of the heat shock protein family.	tag10-2
61300	2	346231	5	NULL	NULL	0	NULL	hsp7O	GP	elevated concentrations of	does not inhibit		significantly			statement 1	Process	induction of			NULL	cultured rat cells	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_6	7935376	In addition, elevated concentrations of hsp7O alone could not significantly inhibit induction of the DNA-binding activity of endogenous HSF in cultured rat cells, and the induction was also not inhibited in cultured rat cells or Drosophila cells containing elevated levels of all members of the heat shock protein family.	tag10-2
61301	3	346231	5	NULL	NULL	0	NULL	heat shock protein family	GP	elevated levels of;;all members of	does not inhibit					statement 1	Process	induction of			NULL	cultured rat cells	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_6	7935376	In addition, elevated concentrations of hsp7O alone could not significantly inhibit induction of the DNA-binding activity of endogenous HSF in cultured rat cells, and the induction was also not inhibited in cultured rat cells or Drosophila cells containing elevated levels of all members of the heat shock protein family.	tag10-2
61302	4	346231	5	NULL	NULL	NULL	NULL	heat shock protein family	GP	elevated levels of;;all members of	does not inhibit					statement 1	Process	induction of			NULL	Drosophila cells	NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_6	7935376	In addition, elevated concentrations of hsp7O alone could not significantly inhibit induction of the DNA-binding activity of endogenous HSF in cultured rat cells, and the induction was also not inhibited in cultured rat cells or Drosophila cells containing elevated levels of all members of the heat shock protein family.	tag10-2
61303	1	346232	5	NULL	NULL	0	NULL	HSF	GP	active	is deactivated to					HSF	GP	non-DNA-bound			NULL		NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_7	7935376	However, the deactivation of HSF to the non-DNA-binding state after prolonged heat stress or during recovery could be accelerated by increased levels of heat shock proteins.	tag10-2
61304	2	346232	5	NULL	NULL	0	NULL	heat stress	Process	prolonged	leads to					statement 1	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_7	7935376	However, the deactivation of HSF to the non-DNA-binding state after prolonged heat stress or during recovery could be accelerated by increased levels of heat shock proteins.	tag10-2
61305	3	346232	5	NULL	NULL	0	NULL	heat shock proteins	GP	increased levels of	accelerates					HSF	GP	recovery of;;deactivated			NULL		NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_7	7935376	However, the deactivation of HSF to the non-DNA-binding state after prolonged heat stress or during recovery could be accelerated by increased levels of heat shock proteins.	tag10-2
61306	1	346233	5	NULL	NULL	0	NULL	heat shock proteins	GP	level of	affects		may			HSF trimers	GP	rate of;;disassembly of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_8	7935376	Hence, the level of heat shock proteins may affect the rate of disassembly of HSF trimers, but another mechanism, as yet undefined, appears to control the onset of the oligomeric transitions.	tag10-2
61307	1	346234	5	NULL	NULL	0	NULL	organisms	Organism		respond to					temperature		elevated			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_9	7935376	Organisms respond to elevated temperatures and to a variety of chemical inducers by rapidly inducing the synthesis of the heat shock proteins (26, 27, 33, 35).	tag10-2
61308	2	346234	5	NULL	NULL	0	NULL	organisms	Organism		induce		rapidly			heat shock proteins	GP	synthesis of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_9	7935376	Organisms respond to elevated temperatures and to a variety of chemical inducers by rapidly inducing the synthesis of the heat shock proteins (26, 27, 33, 35).	tag10-2
61309	3	346234	5	NULL	NULL	0	NULL	statement 1	Process		leads to					statement 2	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_9	7935376	Organisms respond to elevated temperatures and to a variety of chemical inducers by rapidly inducing the synthesis of the heat shock proteins (26, 27, 33, 35).	tag10-2
61310	4	346234	5	NULL	NULL	0	NULL	organisms	Organism		respond to					chemical inducers	Chemical				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_9	7935376	Organisms respond to elevated temperatures and to a variety of chemical inducers by rapidly inducing the synthesis of the heat shock proteins (26, 27, 33, 35).	tag10-2
61311	5	346234	5	NULL	NULL	0	NULL	statement 4	Process		leads to					statement 2	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_9	7935376	Organisms respond to elevated temperatures and to a variety of chemical inducers by rapidly inducing the synthesis of the heat shock proteins (26, 27, 33, 35).	tag10-2
61312	1	346235	5	NULL	NULL	0	NULL	HSF	GP		is					heat shock factor	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_10	7935376	The regulation of this response in eukaryotes is mediated at the transcriptional level by a preexisting transcriptional activator heat shock factor (HSF), which binds to regulatory heat shock elements (HSEs) present upstream of all heat shock genes (28, 29, 48).	tag10-2
61313	2	346235	5	NULL	NULL	0	NULL	HSEs	NucleicAcid		is					heat shock elements	NucleicAcid				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_10	7935376	The regulation of this response in eukaryotes is mediated at the transcriptional level by a preexisting transcriptional activator heat shock factor (HSF), which binds to regulatory heat shock elements (HSEs) present upstream of all heat shock genes (28, 29, 48).	tag10-2
61314	3	346235	5	NULL	NULL	0	NULL	HSF	GP		bind					HSEs	NucleicAcid				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_10	7935376	The regulation of this response in eukaryotes is mediated at the transcriptional level by a preexisting transcriptional activator heat shock factor (HSF), which binds to regulatory heat shock elements (HSEs) present upstream of all heat shock genes (28, 29, 48).	tag10-2
61315	4	346235	5	NULL	NULL	0	NULL	HSF	GP		is a type of					transcriptional activator	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_10	7935376	The regulation of this response in eukaryotes is mediated at the transcriptional level by a preexisting transcriptional activator heat shock factor (HSF), which binds to regulatory heat shock elements (HSEs) present upstream of all heat shock genes (28, 29, 48).	tag10-2
61316	5	346235	5	NULL	NULL	0	NULL	HSEs	NucleicAcid		is located					heat shock genes	GP	upstream of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_10	7935376	The regulation of this response in eukaryotes is mediated at the transcriptional level by a preexisting transcriptional activator heat shock factor (HSF), which binds to regulatory heat shock elements (HSEs) present upstream of all heat shock genes (28, 29, 48).	tag10-2
61317	1	346236	5	NULL	NULL	0	NULL	HSE	NucleicAcid		interacts with				NGAAN repeats	HSF	GP				NULL		NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_11	7935376	The HSE is composed of contiguous, alternating repeats of the 5-bp sequence NGAAN; three NGAAN repeats are required for high-affinity interaction with HSF (3, 13, 37, 38, 59).	tag10-2
61318	1	346237	5	NULL	NULL	0	NULL	HSF	GP		respond to					heat shock signal 	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_12	7935376	HSF responds to the heat shock signal by the induction of DNAbinding activity and transcriptional competence rather than by increasing its own synthesis (22, 28, 48, 57, 58, 60).	tag10-2
61319	2	346237	5	NULL	NULL	0	NULL	HSF	GP		activates					DNA	NucleicAcid	binding of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_12	7935376	HSF responds to the heat shock signal by the induction of DNAbinding activity and transcriptional competence rather than by increasing its own synthesis (22, 28, 48, 57, 58, 60).	tag10-2
61320	3	346237	5	NULL	NULL	0	NULL	statement 1	Process		leads to					statement 2	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_12	7935376	HSF responds to the heat shock signal by the induction of DNAbinding activity and transcriptional competence rather than by increasing its own synthesis (22, 28, 48, 57, 58, 60).	tag10-2
61321	4	346237	5	NULL	NULL	0	NULL	HSF	GP		induce					transcriptional competence	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_12	7935376	HSF responds to the heat shock signal by the induction of DNAbinding activity and transcriptional competence rather than by increasing its own synthesis (22, 28, 48, 57, 58, 60).	tag10-2
61322	5	346237	5	NULL	NULL	0	NULL	statement 1	Process		leads to					statement 4	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_12	7935376	HSF responds to the heat shock signal by the induction of DNAbinding activity and transcriptional competence rather than by increasing its own synthesis (22, 28, 48, 57, 58, 60).	tag10-2
61323	6	346237	5	NULL	NULL	0	NULL	HSF	GP		does not increase					HSF	GP	synthesis of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_12	7935376	HSF responds to the heat shock signal by the induction of DNAbinding activity and transcriptional competence rather than by increasing its own synthesis (22, 28, 48, 57, 58, 60).	tag10-2
61324	1	346238	5	NULL	NULL	NULL	NULL	HSF	GP		bind		high affinity			HSEs	NucleicAcid				NULL	Drosophila melanogaster	NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_13	7935376	For multicellular eukaryotes such as Drosophila melanogaster, vertebrates, and plants, the first stage of HSF activation involves the acquisition of high-affinity binding to HSEs.	tag10-2
61325	2	346238	5	NULL	NULL	NULL	NULL	statement 1	Process		activates					HSF	GP				NULL	Drosophila melanogaster	NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_13	7935376	For multicellular eukaryotes such as Drosophila melanogaster, vertebrates, and plants, the first stage of HSF activation involves the acquisition of high-affinity binding to HSEs.	tag10-2
67119	3	346238	5	NULL	NULL	0	NULL	HSF	GP		bind		high affinity			HSEs	NucleicAcid				NULL	vertebrates	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_13	7935376	For multicellular eukaryotes such as Drosophila melanogaster, vertebrates, and plants, the first stage of HSF activation involves the acquisition of high-affinity binding to HSEs.	tag10-2
67120	4	346238	5	NULL	NULL	NULL	NULL	statement 3	Process		activates					HSF	GP				NULL	vertebrates	NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_13	7935376	For multicellular eukaryotes such as Drosophila melanogaster, vertebrates, and plants, the first stage of HSF activation involves the acquisition of high-affinity binding to HSEs.	tag10-2
67121	5	346238	5	NULL	NULL	0	NULL	HSF	GP		bind		high affinity			HSEs	NucleicAcid				NULL	plants	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_13	7935376	For multicellular eukaryotes such as Drosophila melanogaster, vertebrates, and plants, the first stage of HSF activation involves the acquisition of high-affinity binding to HSEs.	tag10-2
67122	6	346238	5	NULL	NULL	0	NULL	statement 5	Process		activates					HSF	GP				NULL	plants	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_13	7935376	For multicellular eukaryotes such as Drosophila melanogaster, vertebrates, and plants, the first stage of HSF activation involves the acquisition of high-affinity binding to HSEs.	tag10-2
67123	7	346238	5	NULL	NULL	0	NULL	Drosophila melanogaster	Organism		is a type of					multicellular eukaryote	Organism				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_13	7935376	For multicellular eukaryotes such as Drosophila melanogaster, vertebrates, and plants, the first stage of HSF activation involves the acquisition of high-affinity binding to HSEs.	tag10-2
67124	8	346238	5	NULL	NULL	0	NULL	vertebrates	Organism		is a type of					multicellular eukaryote	Organism				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_13	7935376	For multicellular eukaryotes such as Drosophila melanogaster, vertebrates, and plants, the first stage of HSF activation involves the acquisition of high-affinity binding to HSEs.	tag10-2
67125	9	346238	5	NULL	NULL	0	NULL	plants	Organism		is a type of					multicellular eukaryote	Organism				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_13	7935376	For multicellular eukaryotes such as Drosophila melanogaster, vertebrates, and plants, the first stage of HSF activation involves the acquisition of high-affinity binding to HSEs.	tag10-2
61326	1	346239	5	NULL	NULL	0	NULL	HSF	GP		bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_14	7935376	This stress-inducible binding of HSF to DNA is controlled by a monomer-to-trimer transition of HSF protein (4, 44, 55, 56).	tag10-2
61327	2	346239	5	NULL	NULL	0	NULL	stress	Process		induce					statement 1	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_14	7935376	This stress-inducible binding of HSF to DNA is controlled by a monomer-to-trimer transition of HSF protein (4, 44, 55, 56).	tag10-2
61328	3	346239	5	NULL	NULL	0	NULL	HSF monomer protein	GP		is converted to					HSF trimer protein	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_14	7935376	This stress-inducible binding of HSF to DNA is controlled by a monomer-to-trimer transition of HSF protein (4, 44, 55, 56).	tag10-2
61329	4	346239	5	NULL	NULL	0	NULL	statement 3	Process		controls					statement 1	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_14	7935376	This stress-inducible binding of HSF to DNA is controlled by a monomer-to-trimer transition of HSF protein (4, 44, 55, 56).	tag10-2
61330	1	346240	5	NULL	NULL	0	NULL	HSF monomer	GP	isolated	bind		specifically;;low affinity	DNA-binding domain						NGAAN box	NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_15	7935376	An isolated, monomeric HSF DNA-binding domain is capable of binding specifically to a single NGAAN box, but the affinity of this interaction is relatively low (Kd = 10-7 to 10-8 M) (21).	tag10-2
61331	1	346241	5	NULL	NULL	0	NULL	HSF	GP		undergoes					trimerization	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_16	7935376	Trimerization increases the affinity for the HSE by several orders of magnitude through the assembly of three DNAbinding domains of HSF in one complex, thereby allowing the potential for concurrent interactions with all three NGAAN boxes of the HSE.	tag10-2
61332	1	346242	5	NULL	NULL	0	NULL	HSF trimers	GP		bind					HSE	NucleicAcid				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_17	7935376	The binding of HSF trimers to the HSE is necessary but apparently not sufficient for transactivation of heat shock promoters.	tag10-2
61333	2	346242	5	NULL	NULL	0	NULL	statement 1	Process		is necessary for					heat shock proteins	GP	transactivation of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_17	7935376	The binding of HSF trimers to the HSE is necessary but apparently not sufficient for transactivation of heat shock promoters.	tag10-2
61334	3	346242	5	NULL	NULL	0	NULL	statement 1	Process		is not sufficient for					heat shock proteins	GP	transactivation of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_17	7935376	The binding of HSF trimers to the HSE is necessary but apparently not sufficient for transactivation of heat shock promoters.	tag10-2
61335	1	346243	5	NULL	NULL	0	NULL	HSF	GP		bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_18	7935376	Under certain conditions, binding of mammalian HSF to DNA can be uncoupled from the acquisition of transcriptional activity (17, 20).	tag10-2
61336	1	346244	5	NULL	NULL	0	NULL	HSFs	GP	metazoan	undergoes					secondary activation process	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_19	7935376	It is likely that metazoan HSFs undergo a secondary activation process in addition to the monomer-trimer transition to achieve full competence in transactivation.	tag10-2
61337	2	346244	5	NULL	NULL	0	NULL	HSFs mononer	GP	metazoan	is converted to					HSFs trimer	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_19	7935376	It is likely that metazoan HSFs undergo a secondary activation process in addition to the monomer-trimer transition to achieve full competence in transactivation.	tag10-2
61338	3	346244	5	NULL	NULL	0	NULL	statement 1	Process		is required to achieve					HSF	GP	full competence in transactivation of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_19	7935376	It is likely that metazoan HSFs undergo a secondary activation process in addition to the monomer-trimer transition to achieve full competence in transactivation.	tag10-2
61339	4	346244	5	NULL	NULL	0	NULL	statement 2	Process		is required to achieve					HSF	GP	full competence in transactivation of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_19	7935376	It is likely that metazoan HSFs undergo a secondary activation process in addition to the monomer-trimer transition to achieve full competence in transactivation.	tag10-2
61340	1	346245	5	NULL	NULL	0	NULL	trimeric HSF proteins	GP		bind									cognate sites	NULL	in vivo in Saccharomyces cerevisiae	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_20	7935376	Indeed, regulation at the level ofDNA binding is bypassed in the yeasts Saccharomyces cerevisiae and Kluyveromyces lactis, which possess constitutively trimeric HSF proteins bound to their cognate sites in vivo (16, 18, 49, 50).	tag10-2
61341	2	346245	5	NULL	NULL	0	NULL	trimeric HSF proteins	GP		bind									cognate sites	NULL	in vivo in Kluyveromyces lactis	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_20	7935376	Indeed, regulation at the level ofDNA binding is bypassed in the yeasts Saccharomyces cerevisiae and Kluyveromyces lactis, which possess constitutively trimeric HSF proteins bound to their cognate sites in vivo (16, 18, 49, 50).	tag10-2
61342	1	346246	5	NULL	NULL	0	NULL	heat stress	Process		induce					HSF trimers		transactivation function of;;bound			NULL	S. cerevisiae	NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_21	7935376	For S. cerevisiae, it is the transactivation function of bound HSF trimers which is induced upon heat stress, and this activity is correlated with increased phosphorylation at multiple serine and threonine residues (36, 51).	tag10-2
61343	1	346247	5	NULL	NULL	0	NULL	HSF	GP	S. cerevisiae	is masked by			transactivation domain		HSF	GP	internal region of;;S. cerevisiae			NULL		NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_22	7935376	The transactivation domain of S. cerevisiae HSF and K lactis HSF is masked by an internal region of the protein that includes a conserved heptapeptide sequence; mutations in this sequence lead to constitutive activity (6, 19, 36, 47).	tag10-2
61344	2	346247	5	NULL	NULL	0	NULL	HSF	GP	internal region of;;S. cerevisiae	constitutes					heptapeptide sequence	AminoAcid	conserved			NULL		NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_22	7935376	The transactivation domain of S. cerevisiae HSF and K lactis HSF is masked by an internal region of the protein that includes a conserved heptapeptide sequence; mutations in this sequence lead to constitutive activity (6, 19, 36, 47).	tag10-2
61345	3	346247	5	NULL	NULL	0	NULL	statement 2	Process	mutation of	leads to					HSF	GP	constitutive activity of;;S. cerevisiae			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_22	7935376	The transactivation domain of S. cerevisiae HSF and K lactis HSF is masked by an internal region of the protein that includes a conserved heptapeptide sequence; mutations in this sequence lead to constitutive activity (6, 19, 36, 47).	tag10-2
61346	4	346247	5	NULL	NULL	0	NULL	HSF	GP	K lactis	is masked by			transactivation domain		HSF	GP	internal region of;;K lactis			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_22	7935376	The transactivation domain of S. cerevisiae HSF and K lactis HSF is masked by an internal region of the protein that includes a conserved heptapeptide sequence; mutations in this sequence lead to constitutive activity (6, 19, 36, 47).	tag10-2
61347	5	346247	5	NULL	NULL	0	NULL	HSF	GP	internal region of;;K lactis	constitutes					heptapeptide sequence	AminoAcid	conserved			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_22	7935376	The transactivation domain of S. cerevisiae HSF and K lactis HSF is masked by an internal region of the protein that includes a conserved heptapeptide sequence; mutations in this sequence lead to constitutive activity (6, 19, 36, 47).	tag10-2
61348	6	346247	5	NULL	NULL	0	NULL	statement 5	Process	mutation of	leads to					HSF	GP	constitutive activity of;;K lactis			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_22	7935376	The transactivation domain of S. cerevisiae HSF and K lactis HSF is masked by an internal region of the protein that includes a conserved heptapeptide sequence; mutations in this sequence lead to constitutive activity (6, 19, 36, 47).	tag10-2
61349	1	346249	5	NULL	NULL	0	NULL	HSF	GP		bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_24	7935376	The regulation of metazoan HSF binding to DNA is also under negative control.	tag10-2
61350	1	346251	5	NULL	NULL	0	NULL	cellular factors			dictates					HSF	GP	temperature response of 			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_26	7935376	The role of cellular factors in dictating the temperature response of HSF is underscored by the behavior of human HSF1 when the protein is expressed in Drosophila cells, tobacco protoplasts, and frog oocytes.	tag10-2
61351	1	346252	5	NULL	NULL	0	NULL	HSF1	GP	human	is activated at					host heat shock temperature	QuantityOrMeasure				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_27	7935376	In such heterologous cell environments, human HSF1 is activated at the host heat shock temperature, about 10  C below its induction temperature in human cells (4, 8, 53).	tag10-2
61352	1	346253	5	NULL	NULL	0	NULL	HSF monomer	GP	stability of;;latent	is dependent on					HSF	GP		leucine zipper motif;;C-terminal end		NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_28	7935376	These cellular factors may assist in constraining HSF in a latent, monomeric state whose stability is dependent on the integrity of a leucine zipper motif located in the C-terminal end of the protein (41).	tag10-2
61353	1	346254	5	NULL	NULL	0	NULL	HSF	GP		associate with					hsp7O protein	GP				NULL	in vitro	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_29	7935376	While the mechanism of suppression of HSF trimerization is poorly understood in vivo, recent studies have shown an association between HSF and the hsp7O protein in vitro (1, 5, 34, 46).	tag10-2
61354	1	346255	5	NULL	NULL	0	NULL	HSF	GP		activates					DNA	NucleicAcid	binding of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_30	7935376	This association has led to a model for the regulation of the DNA-binding activity of HSF that is principally related to heat shock-induced changes in the level of hsp7O proteins in the cell.	tag10-2
61355	2	346255	5	NULL	NULL	0	NULL	hsp7O proteins	GP	changes in level of	is induced by					heat shock	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_30	7935376	This association has led to a model for the regulation of the DNA-binding activity of HSF that is principally related to heat shock-induced changes in the level of hsp7O proteins in the cell.	tag10-2
61356	3	346255	5	NULL	NULL	0	NULL	statement 1	Process	regulation of	is related to					statement 2	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_30	7935376	This association has led to a model for the regulation of the DNA-binding activity of HSF that is principally related to heat shock-induced changes in the level of hsp7O proteins in the cell.	tag10-2
61357	1	346256	5	NULL	NULL	0	NULL	HSF	GP		associate with					heat shock proteins	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_31	7935376	In this report, we have investigated the association of HSF with heat shock proteins by means of coimmunoprecipitation experiments.	tag10-2
61358	1	346257	5	NULL	NULL	0	NULL	hsp7O	GP		associate with					HSF	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_32	7935376	We find that hsp7O can be associated with HSF, although the extent of the interaction is the same for both the heat-shocked and the unshocked forms of HSF.	tag10-2
61359	1	346258	5	NULL	NULL	0	NULL	HSF	GP		bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_33	7935376	We also find that neither transfected cells expressing increased levels of hsp70 nor cells previously induced to express the entire complement of heat shock proteins show significant effects on the induction of HSF binding to DNA.	tag10-2
61360	1	346259	5	NULL	NULL	0	NULL	HSF	GP		activates					DNA	NucleicAcid	binding of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_34	7935376	These results do not support a simple model for the DNA-binding activity of HSF solely controlled by changes in the levels of hsp70 or other heat shock proteins.	tag10-2
61361	2	346259	5	NULL	NULL	0	NULL	hsp70	GP	changes in levels of	controls					statement 1	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_34	7935376	These results do not support a simple model for the DNA-binding activity of HSF solely controlled by changes in the levels of hsp70 or other heat shock proteins.	tag10-2
61362	3	346259	5	NULL	NULL	0	NULL	heat shock proteins	GP	changes in level of	controls					statement 1	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_34	7935376	These results do not support a simple model for the DNA-binding activity of HSF solely controlled by changes in the levels of hsp70 or other heat shock proteins.	tag10-2
61363	1	346288	5	NULL	NULL	0	NULL	HSF1	GP		complex with					hsp7O					NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_63	7935376	Immunoprecipitation of HSF1-hsp7O complexes.	tag10-2
61364	1	346301	5	NULL	NULL	0	NULL	HSF1	GP	human	associate with					heat shock proteins					NULL	normal HeLa cells	NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_76	7935376	Association of human HSF1 with heat shock proteins in normal and heat-shocked HeLa cells.	tag10-2
61365	2	346301	5	NULL	NULL	0	NULL	HSF1	GP	human	associate with					heat shock proteins	GP				NULL	heat-shocked HeLa cells	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_76	7935376	Association of human HSF1 with heat shock proteins in normal and heat-shocked HeLa cells.	tag10-2
61366	1	346307	5	NULL	NULL	0	NULL	heat shock			effects		potentially			HSF1	GP	phosphorylation state of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_82	7935376	(B) Effect of heat shock on the phosphorylation state of human HSF1.	tag10-2
61367	1	346310	5	NULL	NULL	0	NULL	cellular proteins	GP	radiolabelled	associate with					hHSF1	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_85	7935376	(C) Radiolabeled cellular proteins associating with human HSF1 (hHSF1).	tag10-2
61368	2	346310	5	NULL	NULL	0	NULL	hHSF1	GP		is					human HSF1	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_85	7935376	(C) Radiolabeled cellular proteins associating with human HSF1 (hHSF1).	tag10-2
61369	1	346324	5	NULL	NULL	0	NULL	HSF1	GP		associate with					70-kDa stress proteins	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_99	7935376	RESULTS  Association of HSF1 with 70-kDa stress proteins under normal and heat-shocked conditions.	tag10-2
61370	1	346325	5	NULL	NULL	0	NULL	70-kDa stress proteins	GP		associate with		may			HSF1	GP	human			NULL	HeLa cells	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_100	7935376	We analyzed the association of the 70-kDa stress proteins with human HSF1, the major heat shock-inducible HSF species in HeLa cells (40), using antiserum specific for human HSF1 in a coimmunoprecipitation assay.	tag10-2
61371	1	346328	5	NULL	NULL	0	NULL	HSF1	GP		undergoes					proteolysis	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_103	7935376	As previously reported (23), human HSF1 migrates as a tight cluster of bands whose mobility after heat shock is retarded (Fig. 1A; this sample shows some proteolysis of HSF1).	tag10-2
61372	1	346329	5	NULL	NULL	0	NULL	HSF	GP		undergoes					phosphorylation	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_104	7935376	This change in the electrophoretic mobility of HSF after heat stress is associated with an increase in phosphorylation of the protein (Fig. 1B).	tag10-2
61373	1	346330	5	NULL	NULL	0	NULL	hsc70	GP		bind					HSF1	GP	human			NULL	HeLa cells	NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_105	7935376	We observed that both hsc70 and hsp7O from HeLa cells coimmunoprecipitated with human HSF1, as revealed by closely spaced doublet bands that react with the N27 antibody (Fig. 1A).	tag10-2
61374	2	346330	5	NULL	NULL	0	NULL	hsp7O	GP		bind					HSF1	GP	human			NULL	HeLa cells	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_105	7935376	We observed that both hsc70 and hsp7O from HeLa cells coimmunoprecipitated with human HSF1, as revealed by closely spaced doublet bands that react with the N27 antibody (Fig. 1A).	tag10-2
61375	1	346331	5	NULL	NULL	0	NULL	70-kDa isoform	GP		is expressed in		significantly			primate cells	Cell				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_106	7935376	hsp7O, the lower band of the doublet, was specifically revealed with the C92 antibody; this stress-inducible 70-kDa isoform is expressed at a significant level in primate cells independent of heat stress (32, 54).	tag10-2
61376	2	346331	5	NULL	NULL	0	NULL	statement 1	Process		is independent of					heat stress					NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_106	7935376	hsp7O, the lower band of the doublet, was specifically revealed with the C92 antibody; this stress-inducible 70-kDa isoform is expressed at a significant level in primate cells independent of heat stress (32, 54).	tag10-2
61377	1	346332	5	NULL	NULL	0	NULL	hsp9O	GP		does not bind					HSF1	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_107	7935376	Precipitation of hsp7O or hsc70 was not observed when preimmune serum was used, and another heat shock protein, hsp9O, was not observed to coimmunoprecipitate with HSF1.	tag10-2
61378	1	346333	5	NULL	NULL	0	NULL	70-kDa stress protein		constitutive;;inducible forms of	associate with		specifically			HSF1	GP				NULL	normal HeLa cells	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_108	7935376	The data indicate that both the constitutive and inducible forms of the 70-kDa stress protein associate specifically with HSF1 in normal and heat-treated HeLa cells.	tag10-2
61379	2	346333	5	NULL	NULL	0	NULL	70-kDa stress protein	GP	constitutive;;inducible forms of	associate with		specifically			HSF1	GP				NULL	heat-treated HeLa cells	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_108	7935376	The data indicate that both the constitutive and inducible forms of the 70-kDa stress protein associate specifically with HSF1 in normal and heat-treated HeLa cells.	tag10-2
61380	1	346334	5	NULL	NULL	0	NULL	70-kDa species	GP	32S-labeled	bind					HSF1	GP				NULL	unshocked HeLa cells labeled with [35S]methionine	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_109	7935376	Consistent with these findings, a 32S-labeled 70-kDa species was also found to coimmunoprecipitate with HSF1 when unshocked and heatshocked HeLa cells labeled with [35S]methionine were analyzed (Fig. 1C).	tag10-2
61381	2	346334	5	NULL	NULL	0	NULL	70-kDa species	GP	32S-labeled	bind					HSF1	GP				NULL	heatshocked HeLa cells labeled with [35S]methionine	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_109	7935376	Consistent with these findings, a 32S-labeled 70-kDa species was also found to coimmunoprecipitate with HSF1 when unshocked and heatshocked HeLa cells labeled with [35S]methionine were analyzed (Fig. 1C).	tag10-2
61382	1	346336	5	NULL	NULL	0	NULL	70-kDa stress protein	GP		associate with					HSF1	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_111	7935376	The association between 70-kDa stress protein and HSF1 could not be competed for with unlabeled, exogenous hsc70 protein (Fig. 1D).	tag10-2
61383	2	346336	5	NULL	NULL	0	NULL	hsc70 protein	GP	unlabeled;;exogenous	does not compete with					statement 1	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_111	7935376	The association between 70-kDa stress protein and HSF1 could not be competed for with unlabeled, exogenous hsc70 protein (Fig. 1D).	tag10-2
61384	1	346337	5	NULL	NULL	0	NULL	HSF1	GP		associate with					hsp7O	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_112	7935376	Effect of ATP treatment or prolonged heat shock on the association of HSF1 and hsp7O.	tag10-2
61385	2	346337	5	NULL	NULL	0	NULL	ATP	Chemical	treatment	effects		may			statement 1	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_112	7935376	Effect of ATP treatment or prolonged heat shock on the association of HSF1 and hsp7O.	tag10-2
61386	3	346337	5	NULL	NULL	0	NULL	heat shock		prolonged	effects		may			statement 1	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_112	7935376	Effect of ATP treatment or prolonged heat shock on the association of HSF1 and hsp7O.	tag10-2
61387	1	346338	5	NULL	NULL	0	NULL	HSF1	GP		interacts with		physical			hsp7O	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_113	7935376	To explore the functional significance of the physical interaction between HSF1 and hsp70, we investigated the effects of ATP on the coimmunoprecipitation of the two proteins.	tag10-2
61388	2	346338	5	NULL	NULL	0	NULL	ATP	Chemical		effects		may			statement 1	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_113	7935376	To explore the functional significance of the physical interaction between HSF1 and hsp70, we investigated the effects of ATP on the coimmunoprecipitation of the two proteins.	tag10-2
61389	1	346340	5	NULL	NULL	0	NULL	hsp7O	GP		associate with					HSF1	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_115	7935376	As shown in Fig. 2, the amount of hsp70 associated with HSF1 was not substantially decreased when extracts were treated with ATP.	tag10-2
61390	2	346340	5	NULL	NULL	0	NULL	ATP	Chemical	treatment	does not decrease		substantially			statement 1	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_115	7935376	As shown in Fig. 2, the amount of hsp70 associated with HSF1 was not substantially decreased when extracts were treated with ATP.	tag10-2
61391	1	346342	5	NULL	NULL	0	NULL	HSF1	GP		associate with					hsp7O	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_117	7935376	We also analyzed the possibility of an increased association between HSF1 and hsp70 during prolonged heat stress, which brings about an attenuation of the DNA-binding activity of HSF (2, 42).	tag10-2
61392	2	346342	5	NULL	NULL	0	NULL	heat stress		prolonged	increases		possibly			statement 1	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_117	7935376	We also analyzed the possibility of an increased association between HSF1 and hsp70 during prolonged heat stress, which brings about an attenuation of the DNA-binding activity of HSF (2, 42).	tag10-2
61393	3	346342	5	NULL	NULL	0	NULL	HSF	GP		bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_117	7935376	We also analyzed the possibility of an increased association between HSF1 and hsp70 during prolonged heat stress, which brings about an attenuation of the DNA-binding activity of HSF (2, 42).	tag10-2
61394	4	346342	5	NULL	NULL	0	NULL	statement 2	Process		attenuate					statement 3	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_117	7935376	We also analyzed the possibility of an increased association between HSF1 and hsp70 during prolonged heat stress, which brings about an attenuation of the DNA-binding activity of HSF (2, 42).	tag10-2
61395	1	346343	5	NULL	NULL	0	NULL	HSF1	GP		interacts with					hsp7O	GP				NULL	HeLa cells	NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_118	7935376	When the interaction between HSF1 and hsp7O was analyzed by immunoprecipitation after a continuous heat shock of HeLa cells for 3 h at 42  C, no significant change in the level of association was observed (Fig. 2).	tag10-2
61396	2	346343	5	NULL	NULL	0	NULL	heat shock		continuous	does not change					statement 1	Process	level of			NULL	HeLa cells	NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_118	7935376	When the interaction between HSF1 and hsp7O was analyzed by immunoprecipitation after a continuous heat shock of HeLa cells for 3 h at 42  C, no significant change in the level of association was observed (Fig. 2).	tag10-2
61397	1	346345	5	NULL	NULL	0	NULL	HSF1	GP		activates					DNA	NucleicAcid	binding of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_120	7935376	Hence, the attenuation of DNA-binding activity of HSF1 after prolonged heat shock is apparently not correlated with a measurable increase in the interaction with hsp70 under the conditions of the immunoprecipitation assay.	tag10-2
61398	2	346345	5	NULL	NULL	0	NULL	heat shock		prolonged	attenuate					statement 1	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_120	7935376	Hence, the attenuation of DNA-binding activity of HSF1 after prolonged heat shock is apparently not correlated with a measurable increase in the interaction with hsp70 under the conditions of the immunoprecipitation assay.	tag10-2
61399	3	346345	5	NULL	NULL	0	NULL	HSF1	GP		interacts with					hsp7O	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_120	7935376	Hence, the attenuation of DNA-binding activity of HSF1 after prolonged heat shock is apparently not correlated with a measurable increase in the interaction with hsp70 under the conditions of the immunoprecipitation assay.	tag10-2
61400	4	346345	5	NULL	NULL	0	NULL	statement 2	Process		is not corelated with					statement 3	Process	increase in			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_120	7935376	Hence, the attenuation of DNA-binding activity of HSF1 after prolonged heat shock is apparently not correlated with a measurable increase in the interaction with hsp70 under the conditions of the immunoprecipitation assay.	tag10-2
61401	1	346346	5	NULL	NULL	0	NULL	HSF1	GP		interacts with					70-kDa stress proteins	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_121	7935376	Interaction between HSF1 and 70-kDa stress proteins in vitro does not affect DNA-binding activity.	tag10-2
61402	1	346347	5	NULL	NULL	0	NULL	HSF1	GP	bacterially expressed;;purified	bind					DNA	NucleicAcid				NULL	in vitro	NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_122	7935376	To assess the role of 70-kDa stress proteins on the DNA-binding activity of HSF1 in vitro, purified bovine hsc70 active as uncoating ATPase (15) was incubated with purified, bacterially expressed HSF1.	tag10-2
61403	2	346347	5	NULL	NULL	0	NULL	hsc70	GP	purified;;bovine	plays a role in		may			statement 1	Process				NULL	in vitro	NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_122	7935376	To assess the role of 70-kDa stress proteins on the DNA-binding activity of HSF1 in vitro, purified bovine hsc70 active as uncoating ATPase (15) was incubated with purified, bacterially expressed HSF1.	tag10-2
61405	3	346347	5	NULL	NULL	0	NULL	hsc70	GP		is a type of					70-kDa stress proteins	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_122	7935376	To assess the role of 70-kDa stress proteins on the DNA-binding activity of HSF1 in vitro, purified bovine hsc70 active as uncoating ATPase (15) was incubated with purified, bacterially expressed HSF1.	tag10-2
61404	1	346348	5	NULL	NULL	0	NULL	hsc70	GP		associate with					HSF1- DNA complex	GP				NULL	in vitro	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_123	7935376	As shown by a gel mobility shift assay, the addition of hsc7O caused a retardation in the mobility of the HSF1-DNA complex, suggesting an association between hsc70 and the HSF1- DNA complex in vitro.	tag10-2
61406	1	346349	5	NULL	NULL	0	NULL	HSF1	GP		bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_124	7935376	However, this interaction did not lead to a change in the amount of HSF1 bound to DNA (Fig. 3).	tag10-2
61407	1	346352	5	NULL	NULL	0	NULL	HSF1	GP		interacts with					hsc70	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_127	7935376	The results indicate that there is an interaction between HSF1 and hsc70, but this interaction does not significantly affect the DNA-binding activity of HSF1.	tag10-2
61408	2	346352	5	NULL	NULL	0	NULL	HSF1	GP		activates					DNA	NucleicAcid	binding of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_127	7935376	The results indicate that there is an interaction between HSF1 and hsc70, but this interaction does not significantly affect the DNA-binding activity of HSF1.	tag10-2
61409	3	346352	5	NULL	NULL	0	NULL	statement 1	Process		does not affect		significantly			statement 2	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_127	7935376	The results indicate that there is an interaction between HSF1 and hsc70, but this interaction does not significantly affect the DNA-binding activity of HSF1.	tag10-2
61410	1	346354	5	NULL	NULL	0	NULL	HSF1	GP	human	interacts with					70-kDa stress proteins	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_129	7935376	Effect of ATP and prolonged heat shock on the interaction between human HSF1 and 70-kDa stress proteins.	tag10-2
61411	2	346354	5	NULL	NULL	0	NULL	ATP	Chemical		effects		possibly			statement 1	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_129	7935376	Effect of ATP and prolonged heat shock on the interaction between human HSF1 and 70-kDa stress proteins.	tag10-2
61412	3	346354	5	NULL	NULL	0	NULL	heat shock		prolonged	effects		possibly			statement 1	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_129	7935376	Effect of ATP and prolonged heat shock on the interaction between human HSF1 and 70-kDa stress proteins.	tag10-2
61413	1	346361	5	NULL	NULL	0	NULL	70-kDa stress protein	GP		effects					HSF1	GP	activity of			NULL	in vitro	NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_136	7935376	Effect of 70-kDa stress protein on HSF1 activity in vitro.	tag10-2
61414	1	346366	5	NULL	NULL	0	NULL	HSF1	GP	induction of;;activity of	is not effected by					hsp7O	GP	elevated			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_141	7935376	No effect of elevated hsp7O and heat shock protein levels on induction of HSF1 activity.	tag10-2
61415	2	346366	5	NULL	NULL	0	NULL	HSF1	GP	induction of;;activity of	is not effected by					heat shock protein	GP	level of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_141	7935376	No effect of elevated hsp7O and heat shock protein levels on induction of HSF1 activity.	tag10-2
61416	1	346367	5	NULL	NULL	0	NULL	HSF1	GP	endogenous	activates					DNA	NucleicAcid	binding of			NULL	in vivo rat fibroblast cell line	NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_142	7935376	To assess the role of hsp70 on the DNA-binding activity of HSF1 in vivo, we analyzed the induction of the DNA-binding activity of the endogenous HSF in a rat fibroblast cell line (Ratl) and in the same cell line stably transfected and constitutively expressing the human hsp7O protein (M21 cells [24]).	tag10-2
61417	2	346367	5	NULL	NULL	0	NULL	hsp70	GP	human	plays a role in		possibly			statement 1	Process				NULL	in vivo rat fibroblast cell line	NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_142	7935376	To assess the role of hsp70 on the DNA-binding activity of HSF1 in vivo, we analyzed the induction of the DNA-binding activity of the endogenous HSF in a rat fibroblast cell line (Ratl) and in the same cell line stably transfected and constitutively expressing the human hsp7O protein (M21 cells [24]).	tag10-2
61418	3	346367	5	NULL	NULL	0	NULL	Ratl	Cell		is					rat fibroblast cell line	Cell				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_142	7935376	To assess the role of hsp70 on the DNA-binding activity of HSF1 in vivo, we analyzed the induction of the DNA-binding activity of the endogenous HSF in a rat fibroblast cell line (Ratl) and in the same cell line stably transfected and constitutively expressing the human hsp7O protein (M21 cells [24]).	tag10-2
61419	1	346368	5	NULL	NULL	0	NULL	HSF	GP		activates					DNA	NucleicAcid	binding of			NULL	Ratl cells	NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_143	7935376	We also analyzed the DNA-binding activity of HSF in Ratl cells rendered thermotolerant by heat shock at 45  C for 15 min followed by recovery for 16 h at 37  C.	tag10-2
61420	2	346368	5	NULL	NULL	0	NULL	statement 1	Process		is rendered					thermotolerant	Process				NULL	Ratl cells	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_143	7935376	We also analyzed the DNA-binding activity of HSF in Ratl cells rendered thermotolerant by heat shock at 45  C for 15 min followed by recovery for 16 h at 37  C.	tag10-2
61421	3	346368	5	NULL	NULL	0	NULL	heat shock	QuantityOrMeasure		plays a role in					statement 2	Process				NULL	Ratl cells	NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_143	7935376	We also analyzed the DNA-binding activity of HSF in Ratl cells rendered thermotolerant by heat shock at 45  C for 15 min followed by recovery for 16 h at 37  C.	tag10-2
61422	1	346369	5	NULL	NULL	0	NULL	lTRatl	Cell		is					thermotolerant Ratl cells	Cell				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_144	7935376	These thermotolerant Ratl (lTRatl) cells have elevated levels of the entire complement of heat shock proteins and allow an assessment of whether the increased levels affect the level of the DNA-binding activity in vivo (30).	tag10-2
61423	2	346369	5	NULL	NULL	0	NULL	lTRatl	Cell		contains					heat shock proteins	GP	elevated levels of;;entire complement of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_144	7935376	These thermotolerant Ratl (lTRatl) cells have elevated levels of the entire complement of heat shock proteins and allow an assessment of whether the increased levels affect the level of the DNA-binding activity in vivo (30).	tag10-2
61424	1	346370	5	NULL	NULL	0	NULL	HSF1	GP		activates					DNA	NucleicAcid	binding of			NULL	Ratl cells	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_145	7935376	As shown by the gel mobility shift assay in Fig. 4A, we did not observe significant differences in the levels of DNAbinding activity of HSF1 in extracts prepared from Ratl, TFRatl, or M21 cells after 30 min of heat shock at 42  C.	tag10-2
61425	2	346370	5	NULL	NULL	0	NULL	HSF1	GP		activates					DNA	NucleicAcid	binding of			NULL	TFRatl	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_145	7935376	As shown by the gel mobility shift assay in Fig. 4A, we did not observe significant differences in the levels of DNAbinding activity of HSF1 in extracts prepared from Ratl, TFRatl, or M21 cells after 30 min of heat shock at 42  C.	tag10-2
61426	3	346370	5	NULL	NULL	0	NULL	HSF1	GP		activates					DNA	NucleicAcid	binding of			NULL	M21 cells	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_145	7935376	As shown by the gel mobility shift assay in Fig. 4A, we did not observe significant differences in the levels of DNAbinding activity of HSF1 in extracts prepared from Ratl, TFRatl, or M21 cells after 30 min of heat shock at 42  C.	tag10-2
61427	1	346374	5	NULL	NULL	0	NULL	Ratl cells	Cell	unstressed	contains					hsc70 protein	GP	endogenous			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_149	7935376	As shown in this experiment, unstressed Ratl cells contain endogenous hsc70 protein, while TTRatl cells have the same amount of hsc70 and approximately half that of hsp70 (lower band) accumulated as a result of thermotolerance.	tag10-2
61428	2	346374	5	NULL	NULL	0	NULL	TTRatl cells	Cell		contains					hsc70	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_149	7935376	As shown in this experiment, unstressed Ratl cells contain endogenous hsc70 protein, while TTRatl cells have the same amount of hsc70 and approximately half that of hsp70 (lower band) accumulated as a result of thermotolerance.	tag10-2
61429	3	346374	5	NULL	NULL	0	NULL	TTRatl cells	Cell		contains					hsp70	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_149	7935376	As shown in this experiment, unstressed Ratl cells contain endogenous hsc70 protein, while TTRatl cells have the same amount of hsc70 and approximately half that of hsp70 (lower band) accumulated as a result of thermotolerance.	tag10-2
61430	4	346374	5	NULL	NULL	0	NULL	thermotolerance	Process		leads to					statement 3	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_149	7935376	As shown in this experiment, unstressed Ratl cells contain endogenous hsc70 protein, while TTRatl cells have the same amount of hsc70 and approximately half that of hsp70 (lower band) accumulated as a result of thermotolerance.	tag10-2
61431	1	346375	5	NULL	NULL	0	NULL	M21 cells	Cell		contains					hsc70	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_150	7935376	M21 cells contain a level of hsc70 similar to that of Ratl and lTRat 1 cells, along with a comparable amount of human hsp7o (lower band).	tag10-2
61432	2	346375	5	NULL	NULL	0	NULL	M21 cells	Cell		contains					hsp70	GP	human			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_150	7935376	M21 cells contain a level of hsc70 similar to that of Ratl and lTRat 1 cells, along with a comparable amount of human hsp7o (lower band).	tag10-2
61433	3	346375	5	NULL	NULL	0	NULL	Ratl cells	Cell		contains					hsc70	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_150	7935376	M21 cells contain a level of hsc70 similar to that of Ratl and lTRat 1 cells, along with a comparable amount of human hsp7o (lower band).	tag10-2
61434	4	346375	5	NULL	NULL	0	NULL	lTRat 1 cells	Cell		contains					hsc70	GP				NULL		NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_150	7935376	M21 cells contain a level of hsc70 similar to that of Ratl and lTRat 1 cells, along with a comparable amount of human hsp7o (lower band).	tag10-2
61435	1	346376	5	NULL	NULL	0	NULL	HSF	GP	endogenous	activates					DNA	NucleicAcid	binding of			NULL	M21 cells	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_151	7935376	Thus, an artificial increase in the level of hsp70 protein approximating that found physiologically after a heat stress does not lead to an inhibition of the DNA-binding activity of the endogenous HSF when the M21 cells were subjected to a heat stress.	tag10-2
61436	2	346376	5	NULL	NULL	0	NULL	hsp70 protein	GP	artificial increase in level of	does not inhibit					statement 1	Process				NULL	M21 cells	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_151	7935376	Thus, an artificial increase in the level of hsp70 protein approximating that found physiologically after a heat stress does not lead to an inhibition of the DNA-binding activity of the endogenous HSF when the M21 cells were subjected to a heat stress.	tag10-2
61437	3	346376	5	NULL	NULL	0	NULL	M21 cells	Cell		subjected to					heat stress					NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_151	7935376	Thus, an artificial increase in the level of hsp70 protein approximating that found physiologically after a heat stress does not lead to an inhibition of the DNA-binding activity of the endogenous HSF when the M21 cells were subjected to a heat stress.	tag10-2
61438	4	346376	5	NULL	NULL	0	NULL	statement 3	Process		leads to					statement 2	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_151	7935376	Thus, an artificial increase in the level of hsp70 protein approximating that found physiologically after a heat stress does not lead to an inhibition of the DNA-binding activity of the endogenous HSF when the M21 cells were subjected to a heat stress.	tag10-2
61439	1	346379	5	NULL	NULL	0	NULL	HSF1	GP		activates					DNA	NucleicAcid	binding of			NULL	lTRatl cells	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_154	7935376	The only detectable effect of increased heat shock protein levels on HSF1 activity was a modest decrease (about 30%) in the DNAbinding activity after prolonged heat shock oflTRatl cells for 90 min, while Ratl and M21 cells showed a 10% decrease in the DNA-binding activity of HSF (Fig. 4; also see below).	tag10-2
61440	2	346379	5	NULL	NULL	0	NULL	heat shock		prolonged	decreases		modest			statement 1	Process				NULL	lTRatl cells	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_154	7935376	The only detectable effect of increased heat shock protein levels on HSF1 activity was a modest decrease (about 30%) in the DNAbinding activity after prolonged heat shock oflTRatl cells for 90 min, while Ratl and M21 cells showed a 10% decrease in the DNA-binding activity of HSF (Fig. 4; also see below).	tag10-2
61441	3	346379	5	NULL	NULL	0	NULL	HSF	GP		activates					DNA	NucleicAcid	binding of			NULL	Ratl cells	NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_154	7935376	The only detectable effect of increased heat shock protein levels on HSF1 activity was a modest decrease (about 30%) in the DNAbinding activity after prolonged heat shock oflTRatl cells for 90 min, while Ratl and M21 cells showed a 10% decrease in the DNA-binding activity of HSF (Fig. 4; also see below).	tag10-2
61442	4	346379	5	NULL	NULL	0	NULL	heat shock		prolonged	decreases					statement 3	Process				NULL	Ratl cells	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_154	7935376	The only detectable effect of increased heat shock protein levels on HSF1 activity was a modest decrease (about 30%) in the DNAbinding activity after prolonged heat shock oflTRatl cells for 90 min, while Ratl and M21 cells showed a 10% decrease in the DNA-binding activity of HSF (Fig. 4; also see below).	tag10-2
61443	5	346379	5	NULL	NULL	0	NULL	HSF	GP		activates					DNA	NucleicAcid	binding of			NULL	M21 cells	NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_154	7935376	The only detectable effect of increased heat shock protein levels on HSF1 activity was a modest decrease (about 30%) in the DNAbinding activity after prolonged heat shock oflTRatl cells for 90 min, while Ratl and M21 cells showed a 10% decrease in the DNA-binding activity of HSF (Fig. 4; also see below).	tag10-2
61444	6	346379	5	NULL	NULL	0	NULL	heat shock		prolonged	decreases					statement 5	Process				NULL	M21 cells	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_154	7935376	The only detectable effect of increased heat shock protein levels on HSF1 activity was a modest decrease (about 30%) in the DNAbinding activity after prolonged heat shock oflTRatl cells for 90 min, while Ratl and M21 cells showed a 10% decrease in the DNA-binding activity of HSF (Fig. 4; also see below).	tag10-2
61445	2	346385	5	NULL	NULL	0	NULL	heat shock proteins	GP	elevated expression of	accelerates					statement 1	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_160	7935376	Elevated expression of heat shock proteins accelerates decrease of HSF1 DNA-binding activity during recovery.	tag10-2
61446	1	346385	5	NULL	NULL	0	NULL	HSF1	GP		bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_160	7935376	Elevated expression of heat shock proteins accelerates decrease of HSF1 DNA-binding activity during recovery.	tag10-2
61447	3	346385	5	NULL	NULL	0	NULL	statement 2	Process		occurs during					recovery	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_160	7935376	Elevated expression of heat shock proteins accelerates decrease of HSF1 DNA-binding activity during recovery.	tag10-2
61448	1	346386	5	NULL	NULL	0	NULL	HSF1	GP		bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_161	7935376	Although there was no detectable effect of increased hsp70 and heat shock protein levels on induction of the DNA-binding activity of HSF1, we did observe a reproducible effect of heat shock protein levels on the kinetics of recovery from heat shock.	tag10-2
61449	2	346386	5	NULL	NULL	0	NULL	hsp70	GP	increased levels of	does not effect					statement 1	Process	induction of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_161	7935376	Although there was no detectable effect of increased hsp70 and heat shock protein levels on induction of the DNA-binding activity of HSF1, we did observe a reproducible effect of heat shock protein levels on the kinetics of recovery from heat shock.	tag10-2
61450	3	346386	5	NULL	NULL	0	NULL	heat shock proteins	GP	increased levels of	does not effect					statement 1	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_161	7935376	Although there was no detectable effect of increased hsp70 and heat shock protein levels on induction of the DNA-binding activity of HSF1, we did observe a reproducible effect of heat shock protein levels on the kinetics of recovery from heat shock.	tag10-2
61451	4	346386	5	NULL	NULL	0	NULL	heat shock		recovery from	effects					heat shock proteins	GP	levels of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_161	7935376	Although there was no detectable effect of increased hsp70 and heat shock protein levels on induction of the DNA-binding activity of HSF1, we did observe a reproducible effect of heat shock protein levels on the kinetics of recovery from heat shock.	tag10-2
61452	1	346390	5	NULL	NULL	0	NULL	HSF1	GP		bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_165	7935376	As shown in Fig. 5A, the DNA-binding activity of HSF1 was induced to the same extent in all three cell types.	tag10-2
61453	1	346392	5	NULL	NULL	0	NULL	HSF1	GP		bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_167	7935376	The DNA-binding activities of HSF1 relative to the amount of HSF1 protein in the Ratl and M21 samples (Fig. 5B) were observed to decrease to 50 and 40%, respectively, of maximal levels at 4 h of recovery.	tag10-2
61454	1	346394	5	NULL	NULL	0	NULL	hsp70	GP	increased levels of	effects		modest			HSF	GP	kinetics of;;deactivation of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_169	7935376	These results show that increased levels of hsp70 alone have a modest effect on the kinetics of HSF deactivation, while a full complement of stress proteins can accelerate recovery to the inactive state (Fig. 5D).	tag10-2
61455	1	346395	5	NULL	NULL	0	NULL	PTRatl cells	Cell	increased rate of recovery in	correlates with					HSF1	GP	reversion to hypophosphorylated form of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_170	7935376	This increased rate of recovery in PTRatl cells is also correlated with a reversion to the hypophosphorylated form of HSF1, as shown by the change in SDS-gel mobility (Fig. SB).	tag10-2
61456	1	346396	5	NULL	NULL	0	NULL	HSF	GP		activates					DNA	NucleicAcid	binding of			NULL	Drosophila cells	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_171	7935376	Elevated heat shock protein levels accelerate attenuation but do not block induction of HSF DNA-binding activity in Drosophila cells.	tag10-2
61457	2	346396	5	NULL	NULL	0	NULL	heat shock proteins	GP	elevated levels of	accelerates					statement 1	Process	attenuation of			NULL	Drosophila cells	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_171	7935376	Elevated heat shock protein levels accelerate attenuation but do not block induction of HSF DNA-binding activity in Drosophila cells.	tag10-2
61458	3	346396	5	NULL	NULL	0	NULL	heat shock proteins	GP	elevated levels of	does not block					statement 1	Process	induction of			NULL	Drosophila cells	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_171	7935376	Elevated heat shock protein levels accelerate attenuation but do not block induction of HSF DNA-binding activity in Drosophila cells.	tag10-2
61459	1	346397	5	NULL	NULL	0	NULL	HSF	GP	endogenous	activates					DNA	NucleicAcid	binding of			NULL	Drosophila SL2 cells	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_172	7935376	Since the results presented above could be peculiar to Ratl cells, we analyzed the effects of elevated heat shock protein levels on the DNA-binding activity of the endogenous HSF in Drosophila SL2 cells.	tag10-2
61460	2	346397	5	NULL	NULL	0	NULL	heat shock proteins	GP	elevated levels of	effects		possibly			statement 1	Process				NULL	Drosophila SL2 cells	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_172	7935376	Since the results presented above could be peculiar to Ratl cells, we analyzed the effects of elevated heat shock protein levels on the DNA-binding activity of the endogenous HSF in Drosophila SL2 cells.	tag10-2
61461	1	346398	5	NULL	NULL	0	NULL	HSF	GP	Drosophila	activates					DNA	NucleicAcid	binding of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_173	7935376	We first investigated the effects of prolonged heat shock on the DNA-binding activity of Drosophila HSF.	tag10-2
61462	2	346398	5	NULL	NULL	0	NULL	heat shock		prolonged	effects		possibly			statement 1	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_173	7935376	We first investigated the effects of prolonged heat shock on the DNA-binding activity of Drosophila HSF.	tag10-2
61463	1	346402	5	NULL	NULL	0	NULL	heat shock proteins	GP	elevated levels of	effects		potentially			HSF	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_177	7935376	Thus, the potential effects of elevated heat shock protein levels are operative on HSF only under moderate heat stress.	tag10-2
61464	2	346402	5	NULL	NULL	0	NULL	statement 1	Process		occurs during		only			heat stress	Process	moderate			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_177	7935376	Thus, the potential effects of elevated heat shock protein levels are operative on HSF only under moderate heat stress.	tag10-2
61465	1	346403	5	NULL	NULL	0	NULL	HSF	GP	Drosophila	is deactivated under		possibly			stress conditions	Process	moderate			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_178	7935376	To further investigate the kinetics of Drosophila HSF deactivation under moderate stress conditions, we analyzed the DNA-binding activity of HSF in thermotolerant SL2 (TTSL2) cells (which were previously induced to express heat shock proteins with a 20-min incubation at 37.5  C and a 5-h recovery at 22  C).	tag10-2
61466	1	346404	5	NULL	NULL	0	NULL	cycloheximide	Chemical		prevents					heat shock proteins	GP	de novo synthesis of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_179	7935376	Cells were treated with cycloheximide 30 min before the start of the 34.5  C heat shock to prevent de novo synthesis of heat shock proteins in the course of the continuous heat stress.	tag10-2
61467	1	346405	5	NULL	NULL	0	NULL	HSF	GP	Drosophila	activates					DNA	NucleicAcid	binding of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_180	7935376	As shown by the gel shift assay and Western blotting, the DNA binding activity of Drosophila HSF relative to the amount of HSF protein was not significantly affected when TISL2 cells heat shocked for 15 min were compared with nonthermotolerant SL2 cells stressed similarly (Fig. 7A and B).	tag10-2
61468	2	346405	5	NULL	NULL	0	NULL	statement 1	Process		relative to					HSF protein	GP	amount of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_180	7935376	As shown by the gel shift assay and Western blotting, the DNA binding activity of Drosophila HSF relative to the amount of HSF protein was not significantly affected when TISL2 cells heat shocked for 15 min were compared with nonthermotolerant SL2 cells stressed similarly (Fig. 7A and B).	tag10-2
61469	3	346405	5	NULL	NULL	0	NULL	TISL2 cells	Cell	heat shocked	does not effect					statement 2	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_180	7935376	As shown by the gel shift assay and Western blotting, the DNA binding activity of Drosophila HSF relative to the amount of HSF protein was not significantly affected when TISL2 cells heat shocked for 15 min were compared with nonthermotolerant SL2 cells stressed similarly (Fig. 7A and B).	tag10-2
61470	2	346407	5	NULL	NULL	0	NULL	statement 1		faster decay of	in the absence of					cycloheximide	Chemical				NULL	1TSL2 cells	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_182	7935376	A faster decay of the DNA-binding activity of HSF was also observed when 1TSL2 cells were analyzed in the absence of cycloheximide (data not shown).	tag10-2
61471	1	346407	5	NULL	NULL	0	NULL	HSF	GP		activates					DNA	NucleicAcid	binding of			NULL	1TSL2 cells	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_182	7935376	A faster decay of the DNA-binding activity of HSF was also observed when 1TSL2 cells were analyzed in the absence of cycloheximide (data not shown).	tag10-2
61472	1	346408	5	NULL	NULL	0	NULL	HSF	GP	Drosophila	activates					DNA	NucleicAcid	binding of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_183	7935376	Hence, the presence of previously synthesized heat shock proteins is correlated with an increased rate of attenuation but not with an inhibition of the DNA-binding activity of Drosophila HSF.	tag10-2
61473	2	346408	5	NULL	NULL	0	NULL	heat shock proteins	GP	presence of;;previously synthesized	corelates with					statement 1	Process	increased rate of;;attenuation of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_183	7935376	Hence, the presence of previously synthesized heat shock proteins is correlated with an increased rate of attenuation but not with an inhibition of the DNA-binding activity of Drosophila HSF.	tag10-2
61474	3	346408	5	NULL	NULL	0	NULL	heat shock proteins	GP	presence of;;previously synthesized	doet not corelate with					statement 1	Process	inhibition of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_183	7935376	Hence, the presence of previously synthesized heat shock proteins is correlated with an increased rate of attenuation but not with an inhibition of the DNA-binding activity of Drosophila HSF.	tag10-2
61475	1	346410	5	NULL	NULL	0	NULL	HSF	GP		activates					DNA	NucleicAcid	binding of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_185	7935376	(A to C) Accelerated decrease of HSF DNA-binding activity during recovery from heat shock.	tag10-2
61476	2	346410	5	NULL	NULL	0	NULL	statement 1	Process	accelerated decrease of	occurs during					heat shock		recovery from			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_185	7935376	(A to C) Accelerated decrease of HSF DNA-binding activity during recovery from heat shock.	tag10-2
61477	1	346416	5	NULL	NULL	0	NULL	cell	Cell		measures					thermal stress		level of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_191	7935376	DISCUSSION  The intracellular level of free heat shock proteins in general, and the hsp70 protein family in particular, has been suggested to be part of an autoregulatory loop by which the cell measures the level of thermal stress (10, 11).	tag10-2
61478	2	346416	5	NULL	NULL	0	NULL	autoregulatory loop	Process		plays a role in					statement 1	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_191	7935376	DISCUSSION  The intracellular level of free heat shock proteins in general, and the hsp70 protein family in particular, has been suggested to be part of an autoregulatory loop by which the cell measures the level of thermal stress (10, 11).	tag10-2
61479	3	346416	5	NULL	NULL	0	NULL	heat shock proteins	GP	intracellular level of;;free	is a part of		potentially			statement 2	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_191	7935376	DISCUSSION  The intracellular level of free heat shock proteins in general, and the hsp70 protein family in particular, has been suggested to be part of an autoregulatory loop by which the cell measures the level of thermal stress (10, 11).	tag10-2
61480	4	346416	5	NULL	NULL	0	NULL	hsp70 protein family	GP		is a part of		potentially			statement 2	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_191	7935376	DISCUSSION  The intracellular level of free heat shock proteins in general, and the hsp70 protein family in particular, has been suggested to be part of an autoregulatory loop by which the cell measures the level of thermal stress (10, 11).	tag10-2
61481	1	346417	5	NULL	NULL	0	NULL	HSF	GP		bind					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_192	7935376	This autoregulatory loop has been proposed to affect the DNA-binding and trimerization of HSF.	tag10-2
61482	2	346417	5	NULL	NULL	0	NULL	HSF	GP		undergoes					trimerization	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_192	7935376	This autoregulatory loop has been proposed to affect the DNA-binding and trimerization of HSF.	tag10-2
61483	3	346417	5	NULL	NULL	0	NULL	autoregulatory loop	Process		affects		potentially			statement 1	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_192	7935376	This autoregulatory loop has been proposed to affect the DNA-binding and trimerization of HSF.	tag10-2
61484	4	346417	5	NULL	NULL	0	NULL	autoregulatory loop			affects		potentially			statement 2	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_192	7935376	This autoregulatory loop has been proposed to affect the DNA-binding and trimerization of HSF.	tag10-2
61485	1	346418	5	NULL	NULL	0	NULL	70-kDa stress protein	GP		stabilize					HSF monomer	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_193	7935376	Accordingly, the DNA-binding activity of HSF would be suppressed under normal conditions by the constitutive level of free 70-kDa stress protein, which stabilizes the latent HSF monomer.	tag10-2
61486	2	346418	5	NULL	NULL	0	NULL	HSF	GP		activates					DNA	NucleicAcid	binding of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_193	7935376	Accordingly, the DNA-binding activity of HSF would be suppressed under normal conditions by the constitutive level of free 70-kDa stress protein, which stabilizes the latent HSF monomer.	tag10-2
61487	3	346418	5	NULL	NULL	0	NULL	70-kDa stress protein	GP	constitutive level of;;free	suppress					statement 2	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_193	7935376	Accordingly, the DNA-binding activity of HSF would be suppressed under normal conditions by the constitutive level of free 70-kDa stress protein, which stabilizes the latent HSF monomer.	tag10-2
61488	1	346419	5	NULL	NULL	0	NULL	heat shock		onset of	decreases					70-kDa stress protein	GP	level of;;free			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_194	7935376	As a consequence of the decreased level of free 70-kDa stress protein at the onset of heat shock, the monomeric form of HSF is able to trimerize, leading to high-affinity binding to HSEs and the initiation of the pathway for heat shock protein synthesis.	tag10-2
61489	2	346419	5	NULL	NULL	0	NULL	HSF monomer	GP		undergoes					trimerization	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_194	7935376	As a consequence of the decreased level of free 70-kDa stress protein at the onset of heat shock, the monomeric form of HSF is able to trimerize, leading to high-affinity binding to HSEs and the initiation of the pathway for heat shock protein synthesis.	tag10-2
61490	3	346419	5	NULL	NULL	0	NULL	statement 1	Process		leads to					statement 2	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_194	7935376	As a consequence of the decreased level of free 70-kDa stress protein at the onset of heat shock, the monomeric form of HSF is able to trimerize, leading to high-affinity binding to HSEs and the initiation of the pathway for heat shock protein synthesis.	tag10-2
61491	4	346419	5	NULL	NULL	0	NULL	HSF trimer	GP		bind		high affinity			HSEs	NucleicAcid				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_194	7935376	As a consequence of the decreased level of free 70-kDa stress protein at the onset of heat shock, the monomeric form of HSF is able to trimerize, leading to high-affinity binding to HSEs and the initiation of the pathway for heat shock protein synthesis.	tag10-2
61492	5	346419	5	NULL	NULL	0	NULL	statement 2	Process		leads to					statement 4	Process				NULL		NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_194	7935376	As a consequence of the decreased level of free 70-kDa stress protein at the onset of heat shock, the monomeric form of HSF is able to trimerize, leading to high-affinity binding to HSEs and the initiation of the pathway for heat shock protein synthesis.	tag10-2
61493	6	346419	5	NULL	NULL	0	NULL	statement 4	Process		initiates					heat shock protein 	GP	pathway for;;synthesis of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_194	7935376	As a consequence of the decreased level of free 70-kDa stress protein at the onset of heat shock, the monomeric form of HSF is able to trimerize, leading to high-affinity binding to HSEs and the initiation of the pathway for heat shock protein synthesis.	tag10-2
61494	1	346420	5	NULL	NULL	0	NULL	HSF monomers	GP		is in equilibrium with					HSF trimers	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_195	7935376	The ensuing increase in heat shock protein levels drives the equilibrium between HSF monomers and trimers toward the monomeric species, thus reestablishing the inert form of the transcription factor (5, 9, 31, 34).	tag10-2
61495	2	346420	5	NULL	NULL	0	NULL	statement 1	Process		is driven towards					HSF monomers	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_195	7935376	The ensuing increase in heat shock protein levels drives the equilibrium between HSF monomers and trimers toward the monomeric species, thus reestablishing the inert form of the transcription factor (5, 9, 31, 34).	tag10-2
61496	3	346420	5	NULL	NULL	0	NULL	heat shock proteins	GP	increased levels of	is required for					statement 2	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_195	7935376	The ensuing increase in heat shock protein levels drives the equilibrium between HSF monomers and trimers toward the monomeric species, thus reestablishing the inert form of the transcription factor (5, 9, 31, 34).	tag10-2
61497	4	346420	5	NULL	NULL	0	NULL	statement 3			reestablishes					HSF	GP	inert form of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_195	7935376	The ensuing increase in heat shock protein levels drives the equilibrium between HSF monomers and trimers toward the monomeric species, thus reestablishing the inert form of the transcription factor (5, 9, 31, 34).	tag10-2
61498	5	346420	5	NULL	NULL	0	NULL	HSF	GP		is a type of					transcription factor					NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_195	7935376	The ensuing increase in heat shock protein levels drives the equilibrium between HSF monomers and trimers toward the monomeric species, thus reestablishing the inert form of the transcription factor (5, 9, 31, 34).	tag10-2
61499	1	346422	5	NULL	NULL	0	NULL	HSF	GP	Drosophila	activates					DNA	NucleicAcid	binding of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_197	7935376	DNA-binding activity of Drosophila HSF is attenuated during prolonged heat shock.	tag10-2
61500	2	346422	5	NULL	NULL	0	NULL	heat shock		prolonged	attenuate					statement 1	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_197	7935376	DNA-binding activity of Drosophila HSF is attenuated during prolonged heat shock.	tag10-2
61501	1	346425	5	NULL	NULL	0	NULL	HSF	GP		activates					DNA	NucleicAcid	binding of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_200	7935376	A prediction of this model is that an artificial elevation of heat shock proteins to the level observed after heat shock should inhibit induction of the DNA-binding activity of HSF.	tag10-2
61502	2	346425	5	NULL	NULL	0	NULL	heat shock proteins	GP	artificial elevation of	inhibits					statement 1	Process	induction of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_200	7935376	A prediction of this model is that an artificial elevation of heat shock proteins to the level observed after heat shock should inhibit induction of the DNA-binding activity of HSF.	tag10-2
61505	1	346426	5	NULL	NULL	0	NULL	HSF	GP	endogenous	activates					DNA	NucleicAcid	binding of			NULL		NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_201	7935376	Our test of this prediction with rat M21 cells constitutively expressing hsp70 at a level close to that found physiologically after heat shock and with ITRatl cells expressing a full complement of heat shock proteins indicates that elevated concentrations of hsp7O, alone or in combination with the other heat shock proteins, do not significantly block induction of the DNA-binding activity of the endogenous HSF.	tag10-2
61506	2	346426	5	NULL	NULL	0	NULL	hsp7O	GP	elevated concentrations of	does not block		significantly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_201	7935376	Our test of this prediction with rat M21 cells constitutively expressing hsp70 at a level close to that found physiologically after heat shock and with ITRatl cells expressing a full complement of heat shock proteins indicates that elevated concentrations of hsp7O, alone or in combination with the other heat shock proteins, do not significantly block induction of the DNA-binding activity of the endogenous HSF.	tag10-2
61507	3	346426	5	NULL	NULL	0	NULL	heat shock proteins	GP	full complement of	does not block		significantly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_201	7935376	Our test of this prediction with rat M21 cells constitutively expressing hsp70 at a level close to that found physiologically after heat shock and with ITRatl cells expressing a full complement of heat shock proteins indicates that elevated concentrations of hsp7O, alone or in combination with the other heat shock proteins, do not significantly block induction of the DNA-binding activity of the endogenous HSF.	tag10-2
61508	1	346427	5	NULL	NULL	0	NULL	HSF monomers	GP		is in equilibrium with					HSF trimers	GP				NULL	Drosophila TTSL2 cells	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_202	7935376	Similar findings with Drosophila TTSL2 cells suggest that in general,the equilibrium between HSF monomers and trimers is not solely sensitive to changes in the concentration of heat shock proteins and that some other mechanism for controlling trimerization and the DNA-binding activity of HSF must exist.	tag10-2
61509	2	346427	5	NULL	NULL	0	NULL	statement 1	Process		is not solely sensitive to					heat shock proteins	GP	changes in the concentration of			NULL	Drosophila TTSL2 cells	NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_202	7935376	Similar findings with Drosophila TTSL2 cells suggest that in general,the equilibrium between HSF monomers and trimers is not solely sensitive to changes in the concentration of heat shock proteins and that some other mechanism for controlling trimerization and the DNA-binding activity of HSF must exist.	tag10-2
61510	1	346428	5	NULL	NULL	0	NULL	HSF	GP		is converted to					HSF	GP	non-DNA-bound;;inactive			NULL		NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_203	7935376	However, the inactivation of HSF to the non-DNA-binding state is indeed accelerated by the increased levels of heat shock proteins.	tag10-2
61511	2	346428	5	NULL	NULL	0	NULL	heat shock proteins	GP	increased levels of	accelerates					statement 1	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_203	7935376	However, the inactivation of HSF to the non-DNA-binding state is indeed accelerated by the increased levels of heat shock proteins.	tag10-2
61512	1	346429	5	NULL	NULL	0	NULL	heat shock proteins	GP		assist		directly			HSF trimer	GP	disassembly of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_204	7935376	This finding confirms previous reports (34, 39) and suggests that heat shock proteins do assist, directly or indirectly, in the disassembly of the HSF trimer.	tag10-2
61513	2	346429	5	NULL	NULL	0	NULL	heat shock proteins	GP		assist		indirectly			HSF trimer	GP	disassembly of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_204	7935376	This finding confirms previous reports (34, 39) and suggests that heat shock proteins do assist, directly or indirectly, in the disassembly of the HSF trimer.	tag10-2
61514	3	346429	5	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_204	7935376	This finding confirms previous reports (34, 39) and suggests that heat shock proteins do assist, directly or indirectly, in the disassembly of the HSF trimer.	tag10-2
61515	1	346430	5	NULL	NULL	0	NULL	hsp70	GP		is sequestered in					granules	CellComponent				NULL	Drosophila cells	NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_205	7935376	It should be noted that in a previous study, constitutive overexpression of hsp7O in Drosophila cells led to the sequestration of the protein in granules, where it appears to be irreversibly inactivated and unable to contribute to thermoresistance (12).	tag10-2
61516	2	346430	5	NULL	NULL	0	NULL	hsp70	GP	constitutive overexpression of	leads to					statement 1	Process				NULL	Drosophila cells	NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_205	7935376	It should be noted that in a previous study, constitutive overexpression of hsp7O in Drosophila cells led to the sequestration of the protein in granules, where it appears to be irreversibly inactivated and unable to contribute to thermoresistance (12).	tag10-2
61517	3	346430	5	NULL	NULL	0	NULL	hsp70	GP	sequestered	is inactivated in		irreversibly			granules	CellComponent				NULL	Drosophila cells	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_205	7935376	It should be noted that in a previous study, constitutive overexpression of hsp7O in Drosophila cells led to the sequestration of the protein in granules, where it appears to be irreversibly inactivated and unable to contribute to thermoresistance (12).	tag10-2
61518	4	346430	5	NULL	NULL	0	NULL	hsp70	GP	sequestered	does not contribute to					thermoresistance	Process				NULL	Drosophila cells	NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_205	7935376	It should be noted that in a previous study, constitutive overexpression of hsp7O in Drosophila cells led to the sequestration of the protein in granules, where it appears to be irreversibly inactivated and unable to contribute to thermoresistance (12).	tag10-2
61519	1	346431	5	NULL	NULL	0	NULL	hsp70	GP	constitutively expressed	is inactivate in		possibly			M21 cells	Cell	rat			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_206	7935376	While it is plausible that some of the constitutively expressed hsp7O protein in our rat M21 cells is similarly inactivated, most of the protein appears not to be sequestered in granules (25, 42) and is functional in providing thermoresistance (24, 25, 30).	tag10-2
61520	2	346431	5	NULL	NULL	0	NULL	hsp70	GP	most of	is not sequestered in					granules					NULL	rat M21 cells	NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_206	7935376	While it is plausible that some of the constitutively expressed hsp7O protein in our rat M21 cells is similarly inactivated, most of the protein appears not to be sequestered in granules (25, 42) and is functional in providing thermoresistance (24, 25, 30).	tag10-2
61521	3	346431	5	NULL	NULL	0	NULL	statement 2	GP		provides					thermoresistance	Process				NULL	rat M21 cells	NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_206	7935376	While it is plausible that some of the constitutively expressed hsp7O protein in our rat M21 cells is similarly inactivated, most of the protein appears not to be sequestered in granules (25, 42) and is functional in providing thermoresistance (24, 25, 30).	tag10-2
61522	1	346433	5	NULL	NULL	0	NULL	HSF	GP	Drosophila	activates					DNA	NucleicAcid	binding of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_208	7935376	(A to D) Accelerated decrease of the DNA-binding activity of Drosophila HSF in cells containing accumulated heat shock proteins.	tag10-2
61523	2	346433	5	NULL	NULL	0	NULL	cells	Cell		contain					heat shock proteins	GP	accumulated			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_208	7935376	(A to D) Accelerated decrease of the DNA-binding activity of Drosophila HSF in cells containing accumulated heat shock proteins.	tag10-2
61524	3	346433	5	NULL	NULL	0	NULL	statement 1	Process	accelerated decrease of	occurs in					statement 2	Cell				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_208	7935376	(A to D) Accelerated decrease of the DNA-binding activity of Drosophila HSF in cells containing accumulated heat shock proteins.	tag10-2
61525	1	346438	5	NULL	NULL	0	NULL	HSF	GP		activates					DNA	NucleicAcid	binding of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_213	7935376	(E) Graph showing the relative DNAbinding activity of HSF during prolonged heat shock.	tag10-2
61526	2	346438	5	NULL	NULL	0	NULL	statement 1	Process		occurs during					heat shock		prolonged			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_213	7935376	(E) Graph showing the relative DNAbinding activity of HSF during prolonged heat shock.	tag10-2
61527	1	346440	5	NULL	NULL	0	NULL	HSF	GP		interacts with					hsp70	GP				NULL	in vitro	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_215	7935376	Previous studies detecting in vitro interactions between HSF and hsp7O were based on the electrophoretic retardation of HSF-HSE complexes with hsp70-specific antibodies in a gel shift assay and on the analysis of HSF-hsp7O comnplexes on nondenaturing pore gradient gels (1, 5, 34, 46).	tag10-2
61528	1	346441	5	NULL	NULL	0	NULL	HSF	GP		associate with					hsp70	GP				NULL		NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_216	7935376	The gel shift assay also revealed a greater association of HSF with hsp7O upon prolonged heat stress (1).	tag10-2
61529	2	346441	5	NULL	NULL	0	NULL	heat stress		prolonged	leads to					statement 1	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_216	7935376	The gel shift assay also revealed a greater association of HSF with hsp7O upon prolonged heat stress (1).	tag10-2
61530	1	346442	5	NULL	NULL	0	NULL	70-kDa stress protein	GP		coimmunoprecipitates with					HSF	GP				NULL	heat-shocked cells	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_217	7935376	The coimmunoprecipitation of the 70-kDa stress proteins and HSF that we observed in extracts prepared from heat-shocked cells generally confirms these findings and indicates further that the complexes between HSF and hsp70 or hsc7O are most likely formed in the cell prior to the preparation of cell extracts, since the interaction could not be displaced with an excess of (unlabeled) hsc70 protein.	tag10-2
61531	1	346443	5	NULL	NULL	0	NULL	heat stress		increased	does not lead to					HSF-hsp70	GP	increased interaction of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_218	7935376	However, an increased HSF-hsp70 interaction after prolonged heat stress was not observed in our coimmunoprecipitation studies.	tag10-2
61532	1	346444	5	NULL	NULL	0	NULL	HSF	GP		interacts with					hsp70	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_219	7935376	This difference may be related to the different assays used and may imply a separate mode of interaction between HSF and hsp7O that is detectable only by the gel shift assay after prolonged heat stress.	tag10-2
61533	2	346444	5	NULL	NULL	0	NULL	statement 1	Process		occurs after					heat stress	GP	prolonged			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_219	7935376	This difference may be related to the different assays used and may imply a separate mode of interaction between HSF and hsp7O that is detectable only by the gel shift assay after prolonged heat stress.	tag10-2
61534	1	346445	5	NULL	NULL	0	NULL	70-kDa stress protein	GP		interacts with					HSF monomer	GP	latent			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_220	7935376	The interaction observed between the 70-kDa stress proteins and the latent (monomeric) form of HSF is a new finding.	tag10-2
61535	1	346447	5	NULL	NULL	0	NULL	HSF	GP	latent	coimmunoprecipitates with					70-kDa stress protein	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_222	7935376	The coimmunoprecipitation of both latent and active forms of HSF with the 70-kDa stress proteins is not necessarily inconsistent with sedimentation and gel filtration studies from our laboratory suggesting that the two native forms of HSF are composed of solely one and three HSF subunits, respectively.	tag10-2
61536	2	346447	5	NULL	NULL	0	NULL	HSF	GP	active	coimmunoprecipitates with					70-kDa stress protein	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_222	7935376	The coimmunoprecipitation of both latent and active forms of HSF with the 70-kDa stress proteins is not necessarily inconsistent with sedimentation and gel filtration studies from our laboratory suggesting that the two native forms of HSF are composed of solely one and three HSF subunits, respectively.	tag10-2
61537	3	346447	5	NULL	NULL	0	NULL	HSF	GP	native forms of 	is composed of					HSF subunits	GP				NULL		NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_222	7935376	The coimmunoprecipitation of both latent and active forms of HSF with the 70-kDa stress proteins is not necessarily inconsistent with sedimentation and gel filtration studies from our laboratory suggesting that the two native forms of HSF are composed of solely one and three HSF subunits, respectively.	tag10-2
61538	1	346449	5	NULL	NULL	0	NULL	hsp70	GP		interacts with					HSF	GP	latent			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_224	7935376	As with the interaction observed for the activated HSF, the functional implications of the interactions of hsp7O and hsc70 with the latent HSF are unclear, but they might reflect the participation of molecular chaperones in both the assembly and disassembly of HSF trimers.	tag10-2
61539	2	346449	5	NULL	NULL	0	NULL	hsc70	GP		interacts with					HSF	GP	latent			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_224	7935376	As with the interaction observed for the activated HSF, the functional implications of the interactions of hsp7O and hsc70 with the latent HSF are unclear, but they might reflect the participation of molecular chaperones in both the assembly and disassembly of HSF trimers.	tag10-2
61540	3	346449	5	NULL	NULL	0	NULL	molecular chaperones	GP		participates in		might			HSF trimers	GP	assembly of			NULL		NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_224	7935376	As with the interaction observed for the activated HSF, the functional implications of the interactions of hsp7O and hsc70 with the latent HSF are unclear, but they might reflect the participation of molecular chaperones in both the assembly and disassembly of HSF trimers.	tag10-2
61541	4	346449	5	NULL	NULL	0	NULL	molecular chaperones	GP		participates in		might			HSF trimers	GP	disassembly of			NULL		NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_224	7935376	As with the interaction observed for the activated HSF, the functional implications of the interactions of hsp7O and hsc70 with the latent HSF are unclear, but they might reflect the participation of molecular chaperones in both the assembly and disassembly of HSF trimers.	tag10-2
61542	1	346450	5	NULL	NULL	0	NULL	HSF	GP		interacts with					hsp70	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_225	7935376	We detected only a limited effect of ATP on the interaction between HSF and hsp7O.	tag10-2
61543	2	346450	5	NULL	NULL	0	NULL	ATP	Chemical		effects		limited			statement 1	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_225	7935376	We detected only a limited effect of ATP on the interaction between HSF and hsp7O.	tag10-2
61544	1	346452	5	NULL	NULL	0	NULL	hsp70	GP	chaperone action of	utilizes					ATP	Chemical	hydrolysis of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_227	7935376	In contrast, the known chaperone action of hsp70 utilizes ATP hydrolysis to alter the folded state of proteins and to dissociate oligomeric complexes (43).	tag10-2
61545	2	346452	5	NULL	NULL	0	NULL	statement 1	Process		alter					proteins	GP	folded state of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_227	7935376	In contrast, the known chaperone action of hsp70 utilizes ATP hydrolysis to alter the folded state of proteins and to dissociate oligomeric complexes (43).	tag10-2
61546	3	346452	5	NULL	NULL	0	NULL	statement 2	Process		leads to					oligomeric complex	GP	dissociation of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_227	7935376	In contrast, the known chaperone action of hsp70 utilizes ATP hydrolysis to alter the folded state of proteins and to dissociate oligomeric complexes (43).	tag10-2
61547	1	346453	5	NULL	NULL	0	NULL	HSF	GP		interacts with					hsp70	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_228	7935376	Thus, the observed interaction between HSF and hsp70 may only be a relic of a larger chaperone complex that failed to survive cell extraction.	tag10-2
61548	2	346453	5	NULL	NULL	0	NULL	statement 1	Process		is a relic of		may be			chaperone complex	GP	larger			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_228	7935376	Thus, the observed interaction between HSF and hsp70 may only be a relic of a larger chaperone complex that failed to survive cell extraction.	tag10-2
61549	1	346454	5	NULL	NULL	0	NULL	70-kDa stress protein	GP	purified	does not deactivate					HSF	GP				NULL	in vitro	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_229	7935376	This possibility is reinforced by the inability to deactivate HSF in vitro by using purified 70-kDa stress protein, ATP, and HSF trimers purified from a bacterial expression system.	tag10-2
61550	2	346454	5	NULL	NULL	0	NULL	ATP	Chemical		does not deactivate					HSF	GP				NULL	in vitro	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_229	7935376	This possibility is reinforced by the inability to deactivate HSF in vitro by using purified 70-kDa stress protein, ATP, and HSF trimers purified from a bacterial expression system.	tag10-2
61551	3	346454	5	NULL	NULL	0	NULL	HSF trimers	GP	purified	does not deactivate					HSF	GP				NULL	in vitro	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_229	7935376	This possibility is reinforced by the inability to deactivate HSF in vitro by using purified 70-kDa stress protein, ATP, and HSF trimers purified from a bacterial expression system.	tag10-2
61552	1	346455	5	NULL	NULL	0	NULL	ATP	Chemical	presence of	does not dissociate					HSF-hsp7O complexes					NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_230	7935376	A similar resistance of HSF-hsp7O complexes to disassociation in the presence of ATP has been reported (1, 5).	tag10-2
61553	1	346456	5	NULL	NULL	0	NULL	HSF1	GP	endogenous	activates					DNA	NucleicAcid	binding of			NULL	rat M21 cells	NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_231	7935376	Our finding that the induction of the DNA-binding activity of endogenous HSF1 is not inhibited in rat M21 cells constitutively expressing hsp7O is in conflict with a recent report that showed an inhibition of HSF1 in human PEER cells constitutively expressing hsp7O at a comparable level (34).	tag10-2
61554	2	346456	5	NULL	NULL	0	NULL	rat M21 cells	Cell		express		constitutively			hsp70	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_231	7935376	Our finding that the induction of the DNA-binding activity of endogenous HSF1 is not inhibited in rat M21 cells constitutively expressing hsp7O is in conflict with a recent report that showed an inhibition of HSF1 in human PEER cells constitutively expressing hsp7O at a comparable level (34).	tag10-2
61555	3	346456	5	NULL	NULL	0	NULL	statement 1	Process	induction of	is not inhibited in					statement 2	Process				NULL		NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_231	7935376	Our finding that the induction of the DNA-binding activity of endogenous HSF1 is not inhibited in rat M21 cells constitutively expressing hsp7O is in conflict with a recent report that showed an inhibition of HSF1 in human PEER cells constitutively expressing hsp7O at a comparable level (34).	tag10-2
61556	4	346456	5	NULL	NULL	0	NULL	PEER cells	Cell	human	express					hsp70	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_231	7935376	Our finding that the induction of the DNA-binding activity of endogenous HSF1 is not inhibited in rat M21 cells constitutively expressing hsp7O is in conflict with a recent report that showed an inhibition of HSF1 in human PEER cells constitutively expressing hsp7O at a comparable level (34).	tag10-2
61557	5	346456	5	NULL	NULL	0	NULL	HSF1	GP		is inhibited in					statement 4	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_231	7935376	Our finding that the induction of the DNA-binding activity of endogenous HSF1 is not inhibited in rat M21 cells constitutively expressing hsp7O is in conflict with a recent report that showed an inhibition of HSF1 in human PEER cells constitutively expressing hsp7O at a comparable level (34).	tag10-2
61558	1	346458	5	NULL	NULL	0	NULL	HSF1	GP		is induced by					heat stress					NULL	human PEER cells	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_233	7935376	However, in the absence of a direct measurement of HSF1 levels in the extracts of the human PEER cells that were induced by heat stress, it remains difficult to interpret the observed changes in DNAbinding activity (34).	tag10-2
61559	1	346459	5	NULL	NULL	0	NULL	HSF	GP	latent	is converted to					HSF	GP	active;;DNA-bound			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_234	7935376	These differences indicate the necessity for additional investigations to clarify the role of heat shock proteins in the cycling of HSF between latent and active DNA-binding forms.	tag10-2
61560	2	346459	5	NULL	NULL	0	NULL	heat shock proteins	GP		plays a role in		possibly			statement 1	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_234	7935376	These differences indicate the necessity for additional investigations to clarify the role of heat shock proteins in the cycling of HSF between latent and active DNA-binding forms.	tag10-2
61561	1	346460	5	NULL	NULL	0	NULL	70-kDa stress protein	GP		interacts with		functionally			HSF	GP				NULL	S. cerevisiae	0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_235	7935376	In this respect, it should be noted that there is clear genetic evidence for a functional interaction between the 70-kDa stress proteins and HSF in S. cerevisiae (7, 52).	tag10-2
61562	1	346461	5	NULL	NULL	0	NULL	70-kDa stress protein	GP		repress					heat shock promoters	NucleicAcid	activity of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_236	7935376	These studies indicate that the 70-kDa stress proteins are involved in repressing the activity of heat shock promoters by two different pathways.	tag10-2
66657	1	346462	5	NULL	NULL	0	NULL	one pathway	Process		is independent of					HSE	NucleicAcid				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_237	7935376	One pathway is independent of the HSE (and HSF) and involves an adjacent SRS1 (self-regulating sequence) element (52).	tag10-2
66658	2	346462	5	NULL	NULL	0	NULL	one pathway	Process		is independent of					HSF	GP				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_237	7935376	One pathway is independent of the HSE (and HSF) and involves an adjacent SRS1 (self-regulating sequence) element (52).	tag10-2
66659	3	346462	5	NULL	NULL	0	NULL	statement 1	Process		involves					SRS1 element	NucleicAcid	adjacent			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_237	7935376	One pathway is independent of the HSE (and HSF) and involves an adjacent SRS1 (self-regulating sequence) element (52).	tag10-2
66660	4	346462	5	NULL	NULL	0	NULL	SRS1	NucleicAcid		is					self-regulating sequence	NucleicAcid				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_237	7935376	One pathway is independent of the HSE (and HSF) and involves an adjacent SRS1 (self-regulating sequence) element (52).	tag10-2
61563	1	346463	5	NULL	NULL	0	NULL	HSF trimer	GP	yeast	activates					DNA	NucleicAcid	binding of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_238	7935376	The other pathway implicates HSF, but it involves repression of the transcriptional, not the DNA-binding activity of the constitutively trimeric yeast HSF (7).	tag10-2
66665	2	346463	5	NULL	NULL	0	NULL	HSF trimer	GP	yeast	activates					transcription	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_238	7935376	The other pathway implicates HSF, but it involves repression of the transcriptional, not the DNA-binding activity of the constitutively trimeric yeast HSF (7).	tag10-2
66666	3	346463	5	NULL	NULL	0	NULL	other pathway	Process		repress					statement 2	Process				NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_238	7935376	The other pathway implicates HSF, but it involves repression of the transcriptional, not the DNA-binding activity of the constitutively trimeric yeast HSF (7).	tag10-2
66668	4	346463	5	NULL	NULL	NULL	NULL	other pathway	Process		does not repress					statement 1	Process				NULL		NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_238	7935376	The other pathway implicates HSF, but it involves repression of the transcriptional, not the DNA-binding activity of the constitutively trimeric yeast HSF (7).	tag10-2
61564	1	346464	5	NULL	NULL	0	NULL	HSF	GP	activity of	is repressed by		potentially			hsp70	GP				NULL	yeast	NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_239	7935376	Perhaps it is this repression of HSF activity by hsp7O that operates in yeast and multicellular eukaryotes.	tag10-2
61565	2	346464	5	NULL	NULL	0	NULL	HSF	GP	activity of	is repressed by		potentially			hsp70	GP				NULL	multicellular eukaryotes	NULL	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_239	7935376	Perhaps it is this repression of HSF activity by hsp7O that operates in yeast and multicellular eukaryotes.	tag10-2
61566	1	346465	5	NULL	NULL	0	NULL	HSF	GP		activates					DNA	NucleicAcid	binding of			NULL		0	NULL	NULL	NULL	tag10_molcellbiol_14_10_6552_s_240	7935376	A different mechanism may have evolved to control the oligomeric transition and DNA-binding activity of HSF.	tag10-2
73620	1	354663	7	NULL	NULL	0	NULL	Aripiprazole	Chemical		is used in the					schizophrenia	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	Aripiprazole is used to treat schizophrenia, bipolar mania and mixed manic/depressive episodes (as sole or adjunctive therapy) and as adjunctive (add-on) therapy for major depressive disorder.	topic_bd
73621	2	354663	7	NULL	NULL	0	NULL	Aripiprazole	Chemical		is used in the					bipolar mania	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	Aripiprazole is used to treat schizophrenia, bipolar mania and mixed manic/depressive episodes (as sole or adjunctive therapy) and as adjunctive (add-on) therapy for major depressive disorder.	topic_bd
73622	3	354663	7	NULL	NULL	0	NULL	Aripiprazole	Chemical		is used in the					mixed manic/depressive episodes	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Aripiprazole is used to treat schizophrenia, bipolar mania and mixed manic/depressive episodes (as sole or adjunctive therapy) and as adjunctive (add-on) therapy for major depressive disorder.	topic_bd
73623	4	354663	7	NULL	NULL	0	NULL	Aripiprazole	Chemical		is used as					major depressive disorder	MedicalFinding	adjunctive therapy for			NULL		0	NULL	NULL	NULL	NULL	NULL	Aripiprazole is used to treat schizophrenia, bipolar mania and mixed manic/depressive episodes (as sole or adjunctive therapy) and as adjunctive (add-on) therapy for major depressive disorder.	topic_bd
73624	1	354664	7	NULL	NULL	0	NULL	Abilify	Chemical		brand name for					 aripiprazole	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Abilify is a brand name for aripiprazole.	topic_bd
73625	1	354665	7	NULL	NULL	0	NULL	aripiprazole	Chemical		is not associated with					suicide events	MedicalFinding	increased risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	aripiprazole is not associated with an increased risk of suicide events in an inception cohort of patients with ICD-9/ICD-10 codes indicative of schizophrenia or bipolar disorder.	topic_bd
73626	2	354665	7	NULL	NULL	0	NULL	statement 1	Process		occur in					ICD-9/ICD-10 codes	MedicalFinding	inception cohort of patients with			NULL		0	NULL	NULL	NULL	NULL	NULL	aripiprazole is not associated with an increased risk of suicide events in an inception cohort of patients with ICD-9/ICD-10 codes indicative of schizophrenia or bipolar disorder.	topic_bd
73627	3	354665	7	NULL	NULL	0	NULL	ICD-9/ICD-10 codes	MedicalFinding		indicative of					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	aripiprazole is not associated with an increased risk of suicide events in an inception cohort of patients with ICD-9/ICD-10 codes indicative of schizophrenia or bipolar disorder.	topic_bd
73628	4	354665	7	NULL	NULL	NULL	NULL	ICD-9/ICD-10 codes	MedicalFinding		 indicative of					bipolar disorder	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	aripiprazole is not associated with an increased risk of suicide events in an inception cohort of patients with ICD-9/ICD-10 codes indicative of schizophrenia or bipolar disorder.	topic_bd
73629	5	354665	7	NULL	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	aripiprazole is not associated with an increased risk of suicide events in an inception cohort of patients with ICD-9/ICD-10 codes indicative of schizophrenia or bipolar disorder.	topic_bd
73630	1	354666	7	NULL	NULL	0	NULL	 lithium	Chemical		is useful during					manic phase	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The literature suggests that lithium is useful during the acute manic and the maintenance phase.	topic_bd
73631	2	354666	7	NULL	NULL	NULL	NULL	lithium	Chemical		is useful during					maintenance phase	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	The literature suggests that lithium is useful during the acute manic and the maintenance phase.	topic_bd
73632	1	354667	7	NULL	NULL	0	NULL	Depakote	Chemical		is a type of					antiseizure medication	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Depakote is a antiseizure medication which also works to level out moods.	topic_bd
73633	2	354667	7	NULL	NULL	0	NULL	statement 1	Process		works to					level out moods	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Depakote is a antiseizure medication which also works to level out moods.	topic_bd
73634	1	354668	7	NULL	NULL	0	NULL	ECT	Chemical		treatment for		effective			manic symptoms	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Despite its scary reputation, ECT is an effective treatment for manic symptoms.	topic_bd
73635	1	354669	7	NULL	NULL	0	NULL	hypomania	MedicalFinding		is a type of					less-severe mania	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	This less-severe mania is called hypomania, and is a symptom of bipolar ii disorder.	topic_bd
73636	2	354669	7	NULL	NULL	0	NULL	hypomania	MedicalFinding		symptom of					bipolar ii disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	This less-severe mania is called hypomania, and is a symptom of bipolar ii disorder.	topic_bd
73637	1	354670	7	NULL	NULL	0	NULL	IL-12	GP		promotes					cell-mediated immunity	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-12 (IL-12) promotes cell-mediated immunity by inducing Th1 cell differentiation and activation of both T cells and NK cells.	topic_ccc
73638	2	354670	7	NULL	NULL	0	NULL	statement 1	Process		occur by					Th1 cell	Cell	inducing differentiation of			NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-12 (IL-12) promotes cell-mediated immunity by inducing Th1 cell differentiation and activation of both T cells and NK cells.	topic_ccc
73639	3	354670	7	NULL	NULL	0	NULL	statement 1	Process		occur by					T cell	Cell	activation of			NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-12 (IL-12) promotes cell-mediated immunity by inducing Th1 cell differentiation and activation of both T cells and NK cells.	topic_ccc
73640	4	354670	7	NULL	NULL	0	NULL	statement 1	Process		occur by					NK cells	Cell	activation of			NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-12 (IL-12) promotes cell-mediated immunity by inducing Th1 cell differentiation and activation of both T cells and NK cells.	topic_ccc
73641	5	354670	7	NULL	NULL	0	NULL	statement 3	Process		occur along with					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-12 (IL-12) promotes cell-mediated immunity by inducing Th1 cell differentiation and activation of both T cells and NK cells.	topic_ccc
73642	6	354670	7	NULL	NULL	0	NULL	IL-12	GP		is					Interleukin-12	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-12 (IL-12) promotes cell-mediated immunity by inducing Th1 cell differentiation and activation of both T cells and NK cells.	topic_ccc
73643	1	354671	7	NULL	NULL	0	NULL	A20 cells 	Cell		impairs					CD4 T-cell 	Cell	function of			NULL		0	NULL	NULL	NULL	NULL	NULL	By contrast, CD4 T-cell function appeared impaired after immunization with A20 cells alone or mixed with B78H1 cells. Indeed, only CD4(+) T cells from IL-12-treated mice could be restimulated with anti-OX40 monoclonal antibody (mAb) in place of a fourth cellular boost.	topic_ccc
73644	2	354671	7	NULL	NULL	0	NULL	A20 cells mixed withB78H1 cells	Cell		impairs					CD4 T-cell 	Cell	function of			NULL		0	NULL	NULL	NULL	NULL	NULL	By contrast, CD4 T-cell function appeared impaired after immunization with A20 cells alone or mixed with B78H1 cells. Indeed, only CD4(+) T cells from IL-12-treated mice could be restimulated with anti-OX40 monoclonal antibody (mAb) in place of a fourth cellular boost.	topic_ccc
73645	3	354671	7	NULL	NULL	0	NULL	anti-OX40 mAb	GP		restimulate					CD4(+) T cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	By contrast, CD4 T-cell function appeared impaired after immunization with A20 cells alone or mixed with B78H1 cells. Indeed, only CD4(+) T cells from IL-12-treated mice could be restimulated with anti-OX40 monoclonal antibody (mAb) in place of a fourth cellular boost.	topic_ccc
73646	4	354671	7	NULL	NULL	0	NULL	CD4(+) T cells	Cell		is from					 mice	Organism	 IL-12-treated			NULL		0	NULL	NULL	NULL	NULL	NULL	By contrast, CD4 T-cell function appeared impaired after immunization with A20 cells alone or mixed with B78H1 cells. Indeed, only CD4(+) T cells from IL-12-treated mice could be restimulated with anti-OX40 monoclonal antibody (mAb) in place of a fourth cellular boost.	topic_ccc
73647	1	354672	7	NULL	NULL	NULL	NULL	CD8(+) T cells	Cell		produce					IFN-gamma	GP	 tumor-specific			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Moreover, the IL-12-based tumor vaccine induced expansion of tumor-specific interferon-gamma (IFN-gamma)-producing CD8(+) T cells	topic_ccc
73648	2	354672	7	NULL	NULL	0	NULL	IL-12-based tumor vaccine	GP		induce					CD8(+) T cells	Cell	expansion of			NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, the IL-12-based tumor vaccine induced expansion of tumor-specific interferon-gamma (IFN-gamma)-producing CD8(+) T cells	topic_ccc
73649	3	354672	7	NULL	NULL	0	NULL	IFN-gamma	GP		is					interferon-gamma	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, the IL-12-based tumor vaccine induced expansion of tumor-specific interferon-gamma (IFN-gamma)-producing CD8(+) T cells	topic_ccc
73650	1	354673	7	NULL	NULL	0	NULL	IL-12	GP		displays					antitumor properties	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells. This review focuses on anticancer effects of the IL-12 family in preclinical and clinical studies with an emphasis on colorectal cancer.	topic_ccc
73651	2	354673	7	NULL	NULL	0	NULL	CD4+ T cells	Cell		secrete					(IFN)-γ	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells. This review focuses on anticancer effects of the IL-12 family in preclinical and clinical studies with an emphasis on colorectal cancer.	topic_ccc
73652	3	354673	7	NULL	NULL	0	NULL	CD8+ T cells	Cell		secrete					(IFN)-γ	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells. This review focuses on anticancer effects of the IL-12 family in preclinical and clinical studies with an emphasis on colorectal cancer.	topic_ccc
73653	4	354673	7	NULL	NULL	0	NULL	NK cells	Cell		secrete					(IFN)-γ	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells. This review focuses on anticancer effects of the IL-12 family in preclinical and clinical studies with an emphasis on colorectal cancer.	topic_ccc
73654	5	354673	7	NULL	NULL	0	NULL	NK-T cells	Cell		secrete					(IFN)-γ	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells. This review focuses on anticancer effects of the IL-12 family in preclinical and clinical studies with an emphasis on colorectal cancer.	topic_ccc
73655	6	354673	7	NULL	NULL	0	NULL	statement 1	Process		mediated by					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells. This review focuses on anticancer effects of the IL-12 family in preclinical and clinical studies with an emphasis on colorectal cancer.	topic_ccc
73656	7	354673	7	NULL	NULL	0	NULL	statement 1	Process		mediated by					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells. This review focuses on anticancer effects of the IL-12 family in preclinical and clinical studies with an emphasis on colorectal cancer.	topic_ccc
73657	8	354673	7	NULL	NULL	0	NULL	statement 1	Process		mediated by					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells. This review focuses on anticancer effects of the IL-12 family in preclinical and clinical studies with an emphasis on colorectal cancer.	topic_ccc
73658	9	354673	7	NULL	NULL	0	NULL	statement 1	Process		mediated by					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells. This review focuses on anticancer effects of the IL-12 family in preclinical and clinical studies with an emphasis on colorectal cancer.	topic_ccc
73659	10	354673	7	NULL	NULL	0	NULL	NK cells	cell		is					natural killer cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells. This review focuses on anticancer effects of the IL-12 family in preclinical and clinical studies with an emphasis on colorectal cancer.	topic_ccc
73660	1	354674	7	NULL	NULL	NULL	NULL	IL-12	GP		contributes to					tumor eradication	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	 Importantly, IL-12 through IFN- γ -dependent induction of the antiangiogenic factors interferon-inducible protein (IP) 10 and monokine induced by gamma interferon (MIG) contributes to tumor eradication.	topic_ccc
73661	2	354674	7	NULL	NULL	NULL	NULL	MIG	GP		is					monokine induced by gamma interferon	GP				NULL		NULL	NULL	NULL	NULL	NULL	NULL	 Importantly, IL-12 through IFN- γ -dependent induction of the antiangiogenic factors interferon-inducible protein (IP) 10 and monokine induced by gamma interferon (MIG) contributes to tumor eradication.	topic_ccc
73662	3	354674	7	NULL	NULL	0	NULL	 IFN- γ	GP		induce					IP10	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 Importantly, IL-12 through IFN- γ -dependent induction of the antiangiogenic factors interferon-inducible protein (IP) 10 and monokine induced by gamma interferon (MIG) contributes to tumor eradication.	topic_ccc
73663	4	354674	7	NULL	NULL	0	NULL	 IFN- γ	GP		induce					MIG	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 Importantly, IL-12 through IFN- γ -dependent induction of the antiangiogenic factors interferon-inducible protein (IP) 10 and monokine induced by gamma interferon (MIG) contributes to tumor eradication.	topic_ccc
73664	5	354674	7	NULL	NULL	NULL	NULL	statement 1	Process		act through					statement 3	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	 Importantly, IL-12 through IFN- γ -dependent induction of the antiangiogenic factors interferon-inducible protein (IP) 10 and monokine induced by gamma interferon (MIG) contributes to tumor eradication.	topic_ccc
73665	6	354674	7	NULL	NULL	NULL	NULL	statement 1	Process		act through					statement 4	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	 Importantly, IL-12 through IFN- γ -dependent induction of the antiangiogenic factors interferon-inducible protein (IP) 10 and monokine induced by gamma interferon (MIG) contributes to tumor eradication.	topic_ccc
73666	7	354674	7	NULL	NULL	0	NULL	IP 10	GP		is a type of					antiangiogenic factors	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 Importantly, IL-12 through IFN- γ -dependent induction of the antiangiogenic factors interferon-inducible protein (IP) 10 and monokine induced by gamma interferon (MIG) contributes to tumor eradication.	topic_ccc
73667	8	354674	7	NULL	NULL	0	NULL	MIG	GP		is a type of					antiangiogenic factors	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 Importantly, IL-12 through IFN- γ -dependent induction of the antiangiogenic factors interferon-inducible protein (IP) 10 and monokine induced by gamma interferon (MIG) contributes to tumor eradication.	topic_ccc
73668	9	354674	7	NULL	NULL	0	NULL	IP 10	GP		is a type of					 interferon-inducible protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 Importantly, IL-12 through IFN- γ -dependent induction of the antiangiogenic factors interferon-inducible protein (IP) 10 and monokine induced by gamma interferon (MIG) contributes to tumor eradication.	topic_ccc
73669	1	354675	7	NULL	NULL	0	NULL	IL-12	GP		displays					antitumor properties	Process				NULL	murine models of tumorigenesis	0	NULL	NULL	NULL	NULL	NULL	Moreover, in murine models of tumorigenesis, IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells.	topic_ccc
73670	2	354675	7	NULL	NULL	0	NULL	CD4+ T cells	Cell		secrete					(IFN)-γ	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, in murine models of tumorigenesis, IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells.	topic_ccc
73671	3	354675	7	NULL	NULL	0	NULL	CD8+ T cells	Cell		secrete					(IFN)-γ	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, in murine models of tumorigenesis, IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells.	topic_ccc
73672	4	354675	7	NULL	NULL	0	NULL	NK cells	Cell		secrete					(IFN)-γ	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, in murine models of tumorigenesis, IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells.	topic_ccc
73673	5	354675	7	NULL	NULL	0	NULL	NK-T cells	Cell		secrete					(IFN)-γ	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, in murine models of tumorigenesis, IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells.	topic_ccc
73674	6	354675	7	NULL	NULL	0	NULL	statement 1	Process		mediated by					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, in murine models of tumorigenesis, IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells.	topic_ccc
73675	7	354675	7	NULL	NULL	0	NULL	statement 1	Process		mediated by					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, in murine models of tumorigenesis, IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells.	topic_ccc
73676	8	354675	7	NULL	NULL	0	NULL	statement 1	Process		mediated by					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, in murine models of tumorigenesis, IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells.	topic_ccc
73677	9	354675	7	NULL	NULL	0	NULL	statement 1	Process		mediated by					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, in murine models of tumorigenesis, IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells.	topic_ccc
73678	10	354675	7	NULL	NULL	0	NULL	NK cells	Cell		is					natural killer cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, in murine models of tumorigenesis, IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells.	topic_ccc
73679	1	354676	7	NULL	NULL	NULL	NULL	IL12p70	GP	antitumor effects of	mediated via					IFN γ -IP10/MIG-axis	GP				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Similarly to IL12p70, antitumor effects of IL-27 are mediated via the IFN γ -IP10/MIG-axis and tumor-specific increase of cytotoxic T-lymphocyte activity.	topic_ccc
73680	2	354676	7	NULL	NULL	0	NULL	IL-27	GP	antitumor effects of	mediated via					cytotoxic T-lymphocyte activity	Process	tumor-specific increase of			NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly to IL12p70, antitumor effects of IL-27 are mediated via the IFN γ -IP10/MIG-axis and tumor-specific increase of cytotoxic T-lymphocyte activity.	topic_ccc
73681	3	354676	7	NULL	NULL	NULL	NULL	IL-27	GP	antitumor effects of	mediated via					IFN γ -IP10/MIG-axis	GP				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Similarly to IL12p70, antitumor effects of IL-27 are mediated via the IFN γ -IP10/MIG-axis and tumor-specific increase of cytotoxic T-lymphocyte activity.	topic_ccc
73682	4	354676	7	NULL	NULL	0	NULL	IL12p70	GP	antitumor effects of	mediated via					cytotoxic T-lymphocyte activity	Process	tumor-specific increase of			NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly to IL12p70, antitumor effects of IL-27 are mediated via the IFN γ -IP10/MIG-axis and tumor-specific increase of cytotoxic T-lymphocyte activity.	topic_ccc
73683	1	354677	7	NULL	NULL	0	NULL	 IL-27	GP		mimic					IFN- γ	GP	function of			NULL		0	NULL	NULL	NULL	NULL	NULL	 Additionally, IL-27 itself may mimic the function of IFN- γ due to the similarity in usage of JAK/STAT signalling molecules such as STAT1.	topic_ccc
73684	2	354677	7	NULL	NULL	0	NULL	statement 1	Process		due to					STAT1	GP	similarity in usage of			NULL		0	NULL	NULL	NULL	NULL	NULL	 Additionally, IL-27 itself may mimic the function of IFN- γ due to the similarity in usage of JAK/STAT signalling molecules such as STAT1.	topic_ccc
73685	3	354677	7	NULL	NULL	0	NULL	STAT1	GP		is a type of					JAK/STAT signalling molecules	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 Additionally, IL-27 itself may mimic the function of IFN- γ due to the similarity in usage of JAK/STAT signalling molecules such as STAT1.	topic_ccc
73686	1	354678	7	NULL	NULL	0	NULL	IL-23	GP		act as					procancerogenic	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Whether IL-23 acts pro- or anticancerogenic seems to depend on a critical balance of STAT3 signalling in both the tumor and the immune cellular microenvironment of the tumor.	topic_ccc
73687	2	354678	7	NULL	NULL	0	NULL	IL-23	GP		act as					anticancerogenic	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Whether IL-23 acts pro- or anticancerogenic seems to depend on a critical balance of STAT3 signalling in both the tumor and the immune cellular microenvironment of the tumor.	topic_ccc
73688	3	354678	7	NULL	NULL	NULL	NULL	STAT3 signalling	Process		occur in					tumor	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Whether IL-23 acts pro- or anticancerogenic seems to depend on a critical balance of STAT3 signalling in both the tumor and the immune cellular microenvironment of the tumor.	topic_ccc
73689	4	354678	7	NULL	NULL	NULL	NULL	STAT3 signalling	Process		occur in					tumor	MedicalFinding	 immune cellular microenvironment of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Whether IL-23 acts pro- or anticancerogenic seems to depend on a critical balance of STAT3 signalling in both the tumor and the immune cellular microenvironment of the tumor.	topic_ccc
73690	5	354678	7	NULL	NULL	0	NULL	statement 3	Process		is in balance with					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Whether IL-23 acts pro- or anticancerogenic seems to depend on a critical balance of STAT3 signalling in both the tumor and the immune cellular microenvironment of the tumor.	topic_ccc
73691	6	354678	7	NULL	NULL	0	NULL	statement 1	Process		depends on					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Whether IL-23 acts pro- or anticancerogenic seems to depend on a critical balance of STAT3 signalling in both the tumor and the immune cellular microenvironment of the tumor.	topic_ccc
73692	7	354678	7	NULL	NULL	0	NULL	statement 1	Process		depends on					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Whether IL-23 acts pro- or anticancerogenic seems to depend on a critical balance of STAT3 signalling in both the tumor and the immune cellular microenvironment of the tumor.	topic_ccc
73693	8	354678	7	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Whether IL-23 acts pro- or anticancerogenic seems to depend on a critical balance of STAT3 signalling in both the tumor and the immune cellular microenvironment of the tumor.	topic_ccc
73694	1	354679	7	NULL	NULL	NULL	NULL	IL-12	GP	Long-term controlled expression of	is effective against					hepatic colon cancer metastases	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Long-term controlled expression of IL-12 using an HC-Ad vector in combination with oxaliplatin is effective and clinically applicable against hepatic colon cancer metastases.	topic_ccc
73695	2	354679	7	NULL	NULL	0	NULL	IL-12	GP		in combination with					oxaliplatin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term controlled expression of IL-12 using an HC-Ad vector in combination with oxaliplatin is effective and clinically applicable against hepatic colon cancer metastases.	topic_ccc
73696	3	354679	7	NULL	NULL	0	NULL	IL-12	GP	Long-term controlled expression of	clinically applicable against					hepatic colon cancer metastases	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term controlled expression of IL-12 using an HC-Ad vector in combination with oxaliplatin is effective and clinically applicable against hepatic colon cancer metastases.	topic_ccc
73697	1	354680	7	NULL	NULL	NULL	NULL	MZF	Chemical		upregulate					CD80	Cell	expression of			NULL	DCs	NULL	NULL	NULL	NULL	NULL	NULL	 In this study, we demonstrated that MZF upregulated the expression of CD80, CD86, CD83, and MHC II on bone marrow-derived dendritic cells (DCs) and significantly increased interleukin-12 (IL-12) and tumor necrosis factor-alpha production by DCs in a dose-dependent manner.	topic_ccc
73698	2	354680	7	NULL	NULL	NULL	NULL	MZF	Chemical		upregulate					CD86	Cell	expression of			NULL	DCs	NULL	NULL	NULL	NULL	NULL	NULL	 In this study, we demonstrated that MZF upregulated the expression of CD80, CD86, CD83, and MHC II on bone marrow-derived dendritic cells (DCs) and significantly increased interleukin-12 (IL-12) and tumor necrosis factor-alpha production by DCs in a dose-dependent manner.	topic_ccc
73699	3	354680	7	NULL	NULL	NULL	NULL	MZF	Chemical		upregulate					CD83	Cell	expression of			NULL	Dcs	NULL	NULL	NULL	NULL	NULL	NULL	 In this study, we demonstrated that MZF upregulated the expression of CD80, CD86, CD83, and MHC II on bone marrow-derived dendritic cells (DCs) and significantly increased interleukin-12 (IL-12) and tumor necrosis factor-alpha production by DCs in a dose-dependent manner.	topic_ccc
73700	4	354680	7	NULL	NULL	0	NULL	MZF	Chemical		upregulate					MHC II	GP	expression of			NULL	DCs	0	NULL	NULL	NULL	NULL	NULL	 In this study, we demonstrated that MZF upregulated the expression of CD80, CD86, CD83, and MHC II on bone marrow-derived dendritic cells (DCs) and significantly increased interleukin-12 (IL-12) and tumor necrosis factor-alpha production by DCs in a dose-dependent manner.	topic_ccc
73701	5	354680	7	NULL	NULL	0	NULL	DCs	Cell		produce					IL-12	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 In this study, we demonstrated that MZF upregulated the expression of CD80, CD86, CD83, and MHC II on bone marrow-derived dendritic cells (DCs) and significantly increased interleukin-12 (IL-12) and tumor necrosis factor-alpha production by DCs in a dose-dependent manner.	topic_ccc
73702	6	354680	7	NULL	NULL	0	NULL	DCs	Cell		produce					tumor necrosis factor-alpha	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 In this study, we demonstrated that MZF upregulated the expression of CD80, CD86, CD83, and MHC II on bone marrow-derived dendritic cells (DCs) and significantly increased interleukin-12 (IL-12) and tumor necrosis factor-alpha production by DCs in a dose-dependent manner.	topic_ccc
73703	7	354680	7	NULL	NULL	0	NULL	MZF	Chemical		increase		significantly;;dose-dependently			statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 In this study, we demonstrated that MZF upregulated the expression of CD80, CD86, CD83, and MHC II on bone marrow-derived dendritic cells (DCs) and significantly increased interleukin-12 (IL-12) and tumor necrosis factor-alpha production by DCs in a dose-dependent manner.	topic_ccc
73704	8	354680	7	NULL	NULL	0	NULL	MZF	Chemical		increase		significantly;;dose-dependently			statement 6	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 In this study, we demonstrated that MZF upregulated the expression of CD80, CD86, CD83, and MHC II on bone marrow-derived dendritic cells (DCs) and significantly increased interleukin-12 (IL-12) and tumor necrosis factor-alpha production by DCs in a dose-dependent manner.	topic_ccc
73705	9	354680	7	NULL	NULL	0	NULL	DCs	Cell		is					bone marrow-derived dendritic cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	 In this study, we demonstrated that MZF upregulated the expression of CD80, CD86, CD83, and MHC II on bone marrow-derived dendritic cells (DCs) and significantly increased interleukin-12 (IL-12) and tumor necrosis factor-alpha production by DCs in a dose-dependent manner.	topic_ccc
73706	10	354680	7	NULL	NULL	0	NULL	IL-12	GP		is					interleukin-12	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 In this study, we demonstrated that MZF upregulated the expression of CD80, CD86, CD83, and MHC II on bone marrow-derived dendritic cells (DCs) and significantly increased interleukin-12 (IL-12) and tumor necrosis factor-alpha production by DCs in a dose-dependent manner.	topic_ccc
73707	1	354681	5	NULL	NULL	0	NULL	SHANK3	GP		is a type of					synaptic scaffolding protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the gene encoding the synaptic scaffolding protein SHANK3 are associated with autism spectrum disorders	topic_aut
73708	2	354681	5	NULL	NULL	0	NULL	SHANK3	GP	mutation of	is associated with					autism spectrum disorders	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the gene encoding the synaptic scaffolding protein SHANK3 are associated with autism spectrum disorders	topic_aut
73709	1	354682	5	NULL	NULL	0	NULL	NLGN4 Gene	GP		is a member of					Neuroligin family	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	X-Linked Mental Retardation and Autism Are Associated with a Mutation in the NLGN4 Gene, a Member of the Neuroligin Family	topic_aut
73710	2	354682	5	NULL	NULL	0	NULL	X-Linked Mental Retardation	MedicalFinding		is associated with					NLGN4 Gene	GP	mutation of			NULL		0	NULL	NULL	NULL	NULL	NULL	X-Linked Mental Retardation and Autism Are Associated with a Mutation in the NLGN4 Gene, a Member of the Neuroligin Family	topic_aut
73711	3	354682	5	NULL	NULL	0	NULL	autism	MedicalFinding		is associated with					NLGN4 Gene	GP	mutation of			NULL		0	NULL	NULL	NULL	NULL	NULL	X-Linked Mental Retardation and Autism Are Associated with a Mutation in the NLGN4 Gene, a Member of the Neuroligin Family	topic_aut
73712	1	354683	5	NULL	NULL	0	NULL	toxoplasmosis	MedicalFinding		is linked to		most likely			schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Dr. Milton H. McAllister, professor of pathobiology in the College of Veterinary Medicine at the University of Illinois at Urbana-Champaign, recently announced the strong likelihood of a link between toxoplasmosis and schizophrenia.	topic_sch
73713	1	354684	5	NULL	NULL	NULL	NULL	fra(X)	MedicalFinding		is associated with		significantly			autism	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	With an overall 7.7% frequency of fra(X) among autistic males and an estimated 12.3% of autism among fra(X) males, we conclude there is likely to be a significant association of fra(X) with autism	topic_aut
73715	1	354686	5	NULL	NULL	0	NULL	rs3943552 T allele	NucleicAcid		is a type of					SNP	NucleicAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	Association of the SNP rs3943552 T allele in the GLI2 gene with TD was observed in a subsample of Ashkenazi Jewish patients (N = 96, P = 0.018; P = 6.2 × 10(-5) in the CATIE sample).	topic_sch
73716	2	354686	5	NULL	NULL	0	NULL	rs3943552 T allele	NucleicAcid		is present in					GLI2 gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Association of the SNP rs3943552 T allele in the GLI2 gene with TD was observed in a subsample of Ashkenazi Jewish patients (N = 96, P = 0.018; P = 6.2 × 10(-5) in the CATIE sample).	topic_sch
73717	3	354686	5	NULL	NULL	NULL	NULL	statement 2	NucleicAcid		is associated with					TD	MedicalFinding				NULL	Ashkenazi Jewish patients	NULL	NULL	NULL	NULL	NULL	NULL	Association of the SNP rs3943552 T allele in the GLI2 gene with TD was observed in a subsample of Ashkenazi Jewish patients (N = 96, P = 0.018; P = 6.2 × 10(-5) in the CATIE sample).	topic_sch
73718	1	354687	5	NULL	NULL	0	NULL	GLI2 gene	GP		encodes					transcription factor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The GLI2 gene encodes a transcription factor that participates in the development of the dopaminergic system during embryogenesis.	topic_sch
73719	2	354687	5	NULL	NULL	0	NULL	GLI2 gene	GP		participates in					dopaminergic system	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The GLI2 gene encodes a transcription factor that participates in the development of the dopaminergic system during embryogenesis.	topic_sch
73720	3	354687	5	NULL	NULL	0	NULL	statement 2	Process		occurs during					embryogenesis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The GLI2 gene encodes a transcription factor that participates in the development of the dopaminergic system during embryogenesis.	topic_sch
73721	1	354688	5	NULL	NULL	0	NULL	central serotonergic transmission	Process	dysfunctions of	is involved in		may be			schizophrenia	MedicalFinding	development of			NULL		0	NULL	NULL	NULL	NULL	NULL	Based on the evidence from neurobiological and pharmacological research, dysfunctions in central serotonergic transmission may be involved in the development of schizophrenia. 	topic_sch
73722	1	354689	5	NULL	NULL	0	NULL	TPH2	GP		is					Tryptophan hydroxylase 2	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Tryptophan hydroxylase 2 (TPH2), a newly identified isoform of tryptophan hydroxylase (the rate limiting enzyme in the biosynthesis of serotonin), regulates the brain-specific serotonin synthesis.	topic_sch
73723	2	354689	5	NULL	NULL	0	NULL	TPH2	GP		is an isoform of					tryptophan hydroxylase	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Tryptophan hydroxylase 2 (TPH2), a newly identified isoform of tryptophan hydroxylase (the rate limiting enzyme in the biosynthesis of serotonin), regulates the brain-specific serotonin synthesis.	topic_sch
73724	3	354689	5	NULL	NULL	0	NULL	tryptophan hydroxylase	GP		acts as					rate limiting enzyme	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Tryptophan hydroxylase 2 (TPH2), a newly identified isoform of tryptophan hydroxylase (the rate limiting enzyme in the biosynthesis of serotonin), regulates the brain-specific serotonin synthesis.	topic_sch
73725	4	354689	5	NULL	NULL	0	NULL	statement 3	Process		plays a role in					serotonin	Chemical	biosynthesis of			NULL		0	NULL	NULL	NULL	NULL	NULL	Tryptophan hydroxylase 2 (TPH2), a newly identified isoform of tryptophan hydroxylase (the rate limiting enzyme in the biosynthesis of serotonin), regulates the brain-specific serotonin synthesis.	topic_sch
73726	5	354689	5	NULL	NULL	0	NULL	serotonin	Chemical	synthesis of	is specific to					brain	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Tryptophan hydroxylase 2 (TPH2), a newly identified isoform of tryptophan hydroxylase (the rate limiting enzyme in the biosynthesis of serotonin), regulates the brain-specific serotonin synthesis.	topic_sch
73727	6	354689	5	NULL	NULL	0	NULL	TPH2	GP		regulate					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Tryptophan hydroxylase 2 (TPH2), a newly identified isoform of tryptophan hydroxylase (the rate limiting enzyme in the biosynthesis of serotonin), regulates the brain-specific serotonin synthesis.	topic_sch
73728	1	354691	5	NULL	NULL	0	NULL	TPH2	GP		develops				rs4570625	positive symptoms	PhysicalPhenomenon				NULL	Han Chinese schizophrenic patients	0	NULL	NULL	NULL	NULL	NULL	These results suggest that rs4570625 of TPH2 may play an important role in the development of positive symptoms in Han Chinese schizophrenic patients.	topic_sch
73730	1	354694	5	NULL	NULL	0	NULL	schizophrenia 	MedicalFinding		is associated with					frontotemporal lobar degeneration	Process	behavioral variant of			NULL		0	NULL	NULL	NULL	NULL	NULL	Major psychiatric diseases such as schizophrenia and mood disorders have not been linked to a specific pathology, but their clinical features overlap with some aspects of the behavioral variant of frontotemporal lobar degeneration.	topic_sch
73731	2	354694	5	NULL	NULL	0	NULL	mood disorders	MedicalFinding		is associated with					frontotemporal lobar degeneration	Process	behavioral variant of			NULL		0	NULL	NULL	NULL	NULL	NULL	Major psychiatric diseases such as schizophrenia and mood disorders have not been linked to a specific pathology, but their clinical features overlap with some aspects of the behavioral variant of frontotemporal lobar degeneration.	topic_sch
73732	1	354695	5	NULL	NULL	NULL	NULL	TDP-43	GP	pathological	plays a role in		significant			frontotemporal lobar degeneration	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although the significance of pathological 43-kDa (transactivation response) DNA-binding protein (TDP-43) for frontotemporal lobar degeneration was appreciated only recently, the prevalence of TDP-43 pathology in patients with severe mental illness vs controls has not been systematically addressed.	topic_sch
73733	2	354695	5	NULL	NULL	0	NULL	TDP-43	GP		is					 43-kDa transactivation response DNA-binding protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Although the significance of pathological 43-kDa (transactivation response) DNA-binding protein (TDP-43) for frontotemporal lobar degeneration was appreciated only recently, the prevalence of TDP-43 pathology in patients with severe mental illness vs controls has not been systematically addressed.	topic_sch
73734	2	354697	5	NULL	NULL	0	NULL	GRN variant	GP		is found in					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	A new GRN variant of unknown significance (c.620T>C, p.Met207Thr) was found in 1 patient with schizophrenia with TDP-43 pathology.	topic_sch
73735	1	354697	5	NULL	NULL	0	NULL	schizophrenia patient	GroupOfPeople		contains					TDP-43	GP	pathological			NULL		0	NULL	NULL	NULL	NULL	NULL	A new GRN variant of unknown significance (c.620T>C, p.Met207Thr) was found in 1 patient with schizophrenia with TDP-43 pathology.	topic_sch
73736	1	354698	5	NULL	NULL	NULL	NULL	psychiatric patients	GroupOfPeople		is prone to					vascular risk	PhysicalPhenomenon	increased			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Evidence suggests that psychiatric patients are at an increased vascular risk. 	topic_sch
73737	1	354699	5	NULL	NULL	NULL	NULL	sRAGE	GP		is associated with					atherothrombosis	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this exploratory pilot study, we hypothesized that low levels of the soluble receptor for advanced glycation endproducts (sRAGE) might be found in psychiatric patients due to its association with atherothrombosis.	topic_sch
73738	2	354699	5	NULL	NULL	0	NULL	sRAGE	GP		is					soluble receptor for advanced glycation endproducts	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	In this exploratory pilot study, we hypothesized that low levels of the soluble receptor for advanced glycation endproducts (sRAGE) might be found in psychiatric patients due to its association with atherothrombosis.	topic_sch
73739	3	354699	5	NULL	NULL	0	NULL	sRAGE	GP	low levels of	is found in		might be			psychiatric patients	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	In this exploratory pilot study, we hypothesized that low levels of the soluble receptor for advanced glycation endproducts (sRAGE) might be found in psychiatric patients due to its association with atherothrombosis.	topic_sch
73740	1	354701	5	NULL	NULL	0	NULL	sRAGE	GP	reduced serum	contribute to					cardiovascular risk	MedicalFinding	increased			NULL	schizophrenia	0	NULL	NULL	NULL	NULL	NULL	Although subject to future confirmation, our findings suggest that the reduced serum sRAGE may contribute to increased cardiovascular risk in schizophrenia and major depression.	topic_sch
73741	2	354701	5	NULL	NULL	0	NULL	sRAGE	GP	reduced serum	contribute to					cardiovascular risk	MedicalFinding	increased			NULL	major depression	0	NULL	NULL	NULL	NULL	NULL	Although subject to future confirmation, our findings suggest that the reduced serum sRAGE may contribute to increased cardiovascular risk in schizophrenia and major depression.	topic_sch
73742	1	354702	5	NULL	NULL	0	NULL	AZD2624	Chemical		is a antagonist of					NK3 receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	AZD2624 was pharmacologically characterized as a NK3 receptor antagonist intended for treatment of schizophrenia.	topic_sch
73743	2	354702	5	NULL	NULL	0	NULL	AZD2624	Chemical		is intended for					schizophrenia	MedicalFinding	treatment of 			NULL		0	NULL	NULL	NULL	NULL	NULL	AZD2624 was pharmacologically characterized as a NK3 receptor antagonist intended for treatment of schizophrenia.	topic_sch
73744	1	354703	5	NULL	NULL	NULL	NULL	tardive OGC	MedicalFinding		is related to					amisulpride	Chemical				NULL	young woman with schizophrenia	NULL	NULL	NULL	NULL	NULL	NULL	We report a case of a young woman with schizophrenia who presented with tardive OGC related to amisulpride.	topic_sch
73745	1	354704	5	NULL	NULL	0	NULL	ZNF804A	Chemical		delinates					schizophrenia subtype	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	These data are consistent with our earlier behavioral data and suggest that ZNF804A is delineating a schizophrenia subtype characterized by relatively intact brain volume. 	topic_sch
73746	2	354704	5	NULL	NULL	0	NULL	schizophrenia subtype	MedicalFinding		is characterized by					brain volume	PhysicalPhenomenon	relatively intact			NULL		0	NULL	NULL	NULL	NULL	NULL	These data are consistent with our earlier behavioral data and suggest that ZNF804A is delineating a schizophrenia subtype characterized by relatively intact brain volume. 	topic_sch
73747	1	354705	5	NULL	NULL	NULL	NULL	ZNF804A variants	GP		increases		weakly			schizophrenia	MedicalFinding	susceptibility to			NULL		NULL	NULL	NULL	NULL	NULL	NULL	These include ZNF804A, TCF4 and NRGN, which contain common variants that weakly increase schizophrenia susceptibility, and NRXN1, in which rare copy number variants have a greater impact on schizophrenia risk. 	topic_sch
73748	2	354705	5	NULL	NULL	0	NULL	TCF4 variants	GP		increases		weakly			schizophrenia	MedicalFinding	susceptibility to			NULL		0	NULL	NULL	NULL	NULL	NULL	These include ZNF804A, TCF4 and NRGN, which contain common variants that weakly increase schizophrenia susceptibility, and NRXN1, in which rare copy number variants have a greater impact on schizophrenia risk. 	topic_sch
73749	3	354705	5	NULL	NULL	0	NULL	NRGN variants	GP		increases		weakly			schizophrenia	MedicalFinding	susceptibility to			NULL		0	NULL	NULL	NULL	NULL	NULL	These include ZNF804A, TCF4 and NRGN, which contain common variants that weakly increase schizophrenia susceptibility, and NRXN1, in which rare copy number variants have a greater impact on schizophrenia risk. 	topic_sch
73750	4	354705	5	NULL	NULL	0	NULL	NRXN1 variant	GP		impacts		greatly			schizophrenia 	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	These include ZNF804A, TCF4 and NRGN, which contain common variants that weakly increase schizophrenia susceptibility, and NRXN1, in which rare copy number variants have a greater impact on schizophrenia risk. 	topic_sch
73751	1	354706	5	NULL	NULL	0	NULL	mGluRs	GP	activation of	plays a role in		important			schizophrenia	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	In the meantime, several novel pharmacological strategies, including activation of mGluRs, elevation of synaptic glycine and inhibition of phosphodiesterase 10A, have recently shown promise for the treatment of schizophrenia in clinical trials.	topic_sch
73752	2	354706	5	NULL	NULL	0	NULL	synaptic glycine	AminoAcid	elevation of	plays a role in		important			schizophrenia	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	In the meantime, several novel pharmacological strategies, including activation of mGluRs, elevation of synaptic glycine and inhibition of phosphodiesterase 10A, have recently shown promise for the treatment of schizophrenia in clinical trials.	topic_sch
73753	3	354706	5	NULL	NULL	0	NULL	phosphodiesterase 10A	GP	inhibition of	plays a role in		important			schizophrenia	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	In the meantime, several novel pharmacological strategies, including activation of mGluRs, elevation of synaptic glycine and inhibition of phosphodiesterase 10A, have recently shown promise for the treatment of schizophrenia in clinical trials.	topic_sch
73754	1	354707	5	NULL	NULL	0	NULL	COMT	GP		is					Catechol-O-methyl transferase	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Catechol-O-methyl transferase (COMT) encodes an enzyme involved in the metabolism of dopamine and maps to a commonly deleted region that increases schizophrenia risk. 	topic_sch
73755	2	354707	5	NULL	NULL	0	NULL	COMT	GP		is involved in					dopamine	Chemical	metabolism of			NULL		0	NULL	NULL	NULL	NULL	NULL	Catechol-O-methyl transferase (COMT) encodes an enzyme involved in the metabolism of dopamine and maps to a commonly deleted region that increases schizophrenia risk. 	topic_sch
73756	3	354707	5	NULL	NULL	0	NULL	COMT	GP	deletion of	increases					schizophrenia	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	Catechol-O-methyl transferase (COMT) encodes an enzyme involved in the metabolism of dopamine and maps to a commonly deleted region that increases schizophrenia risk. 	topic_sch
73757	1	354708	5	NULL	NULL	NULL	NULL	rs4680	NucleicAcid		is associated with		significantly			schizophrenia	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two polymorphisms including rs4680 and rs165774 were found to be significantly associated with schizophrenia. 	topic_sch
73758	2	354708	5	NULL	NULL	NULL	NULL	rs165774	NucleicAcid		is associated with		significantly			schizophrenia	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two polymorphisms including rs4680 and rs165774 were found to be significantly associated with schizophrenia. 	topic_sch
73759	3	354708	5	NULL	NULL	0	NULL	rs4680	NucleicAcid		is a type of					polymorphism	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Two polymorphisms including rs4680 and rs165774 were found to be significantly associated with schizophrenia. 	topic_sch
73760	4	354708	5	NULL	NULL	0	NULL	rs165774	NucleicAcid		is a type of					polymorphism	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Two polymorphisms including rs4680 and rs165774 were found to be significantly associated with schizophrenia. 	topic_sch
74508	1	354709	6	NULL	NULL	0	NULL	BRCA1	GP		regulates					cell division	Process	cycle of 			NULL		0	NULL	NULL	NULL	NULL	NULL	Like many other tumor suppressor genes, BRCA1 regulates the cycle of cell division by keeping cells from growing and dividing too rapidly	topic_bc
74509	2	354709	6	NULL	NULL	0	NULL	BRCA1	GP		regulates					cells	Cell	rapid;; growing of			NULL		0	NULL	NULL	NULL	NULL	NULL	Like many other tumor suppressor genes, BRCA1 regulates the cycle of cell division by keeping cells from growing and dividing too rapidly	topic_bc
74510	1	354710	6	NULL	NULL	0	NULL	BRCA2	GP		belongs to					tumor suppressor gene family	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	BRCA2 belongs to the tumor suppressor gene family	topic_bc
74511	1	354711	6	NULL	NULL	0	NULL	BRCA1	GP	mutation of	increases					breast cancer	MedicalFinding	risk of 			NULL		0	NULL	NULL	NULL	NULL	NULL	A woman's risk of developing breast and/or ovarian cancer is greatly increased if she inherits a deleterious (harmful) BRCA1 or BRCA2 mutation. Men with these mutations also have an increased risk of breast cancer. Both men and women who have harmful BRCA1 or BRCA2 mutations may be at increased risk of other cancer	topic_bc
74512	2	354711	6	NULL	NULL	0	NULL	BRCA2	GP	mutation of	increases					breast cancer	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	A woman's risk of developing breast and/or ovarian cancer is greatly increased if she inherits a deleterious (harmful) BRCA1 or BRCA2 mutation. Men with these mutations also have an increased risk of breast cancer. Both men and women who have harmful BRCA1 or BRCA2 mutations may be at increased risk of other cancer	topic_bc
74513	3	354711	6	NULL	NULL	NULL	NULL	BRCA1	GP	mutation of	increases					ovarian cancer	MedicalFinding	risk of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	A woman's risk of developing breast and/or ovarian cancer is greatly increased if she inherits a deleterious (harmful) BRCA1 or BRCA2 mutation. Men with these mutations also have an increased risk of breast cancer. Both men and women who have harmful BRCA1 or BRCA2 mutations may be at increased risk of other cancer	topic_bc
74514	4	354711	6	NULL	NULL	0	NULL	BRCA2	GP	mutation of	increases					ovarian cancer	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	A woman's risk of developing breast and/or ovarian cancer is greatly increased if she inherits a deleterious (harmful) BRCA1 or BRCA2 mutation. Men with these mutations also have an increased risk of breast cancer. Both men and women who have harmful BRCA1 or BRCA2 mutations may be at increased risk of other cancer	topic_bc
74515	1	354712	6	NULL	NULL	0	NULL	colon cancer	MedicalFinding		is linked to					aging	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	There are certain cancers, in particular, that are linked to aging. These include colon, rectal, prostate, pancreas, lung, bladder, stomach and breast cancers.	topic_bc
74516	2	354712	6	NULL	NULL	0	NULL	rectal cancer	MedicalFinding		is linked to					aging	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	There are certain cancers, in particular, that are linked to aging. These include colon, rectal, prostate, pancreas, lung, bladder, stomach and breast cancers.	topic_bc
74517	3	354712	6	NULL	NULL	0	NULL	prostate cancer	MedicalFinding		is linked to					aging	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	There are certain cancers, in particular, that are linked to aging. These include colon, rectal, prostate, pancreas, lung, bladder, stomach and breast cancers.	topic_bc
74518	4	354712	6	NULL	NULL	0	NULL	pancreatic cancer	MedicalFinding		is linked to					aging	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	There are certain cancers, in particular, that are linked to aging. These include colon, rectal, prostate, pancreas, lung, bladder, stomach and breast cancers.	topic_bc
74519	5	354712	6	NULL	NULL	0	NULL	lung cancer	MedicalFinding		is linked to					aging	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	There are certain cancers, in particular, that are linked to aging. These include colon, rectal, prostate, pancreas, lung, bladder, stomach and breast cancers.	topic_bc
74520	6	354712	6	NULL	NULL	0	NULL	Bladder cancer	MedicalFinding		is linked to					aging	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	There are certain cancers, in particular, that are linked to aging. These include colon, rectal, prostate, pancreas, lung, bladder, stomach and breast cancers.	topic_bc
74521	7	354712	6	NULL	NULL	0	NULL	stomach cancer	MedicalFinding		is linked to					aging	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	There are certain cancers, in particular, that are linked to aging. These include colon, rectal, prostate, pancreas, lung, bladder, stomach and breast cancers.	topic_bc
74522	8	354712	6	NULL	NULL	0	NULL	breast cancer	MedicalFinding		is linked to					aging	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	There are certain cancers, in particular, that are linked to aging. These include colon, rectal, prostate, pancreas, lung, bladder, stomach and breast cancers.	topic_bc
74523	1	354713	6	NULL	NULL	0	NULL	women	GroupOfPeople		have					breast	CellComponent	dense			NULL		0	NULL	NULL	NULL	NULL	NULL	Cancer turns up five times more often in women with extremely dense breasts than in those with the most fatty tissue	topic_bc
74524	2	354713	6	NULL	NULL	0	NULL	cancer	MedicalFinding		is more in					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Cancer turns up five times more often in women with extremely dense breasts than in those with the most fatty tissue	topic_bc
74525	1	354714	6	NULL	NULL	0	NULL	post-menopausal hormone therapy	MedicalProcedure		increases 					breast cancer	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	Use of combined post-menopausal hormone therapy increases the risk of getting breast cancer	topic_bc
74526	1	354715	6	NULL	NULL	0	NULL	wine	Food		increases					breast cancer	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	drinking as little as half a glass of wine a day may raise a woman's risk of developing breast cancer	topic_bc
74527	1	354716	6	NULL	NULL	0	NULL	exercise	MentalProcess	vigrous	cuts					breast cancer	MedicalFinding	risk of			NULL	post-menopausal women	0	NULL	NULL	NULL	NULL	NULL	New research from the US suggests that vigorous exercise cuts the risk of breast cancer in post-menopausal women	topic_bc
74528	1	354717	6	NULL	NULL	0	NULL	oxidation	Process		causes					DNA	NucleicAcid	damage to			NULL		0	NULL	NULL	NULL	NULL	NULL	While the importance of ATM function to protect against oxidative DNA damage and during ageing is well described	topic_bc
74529	2	354717	6	NULL	NULL	0	NULL	ATM	GP		protects against					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	While the importance of ATM function to protect against oxidative DNA damage and during ageing is well described	topic_bc
74530	3	354717	6	NULL	NULL	0	NULL	ATM	GP		protects against					ageing	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	While the importance of ATM function to protect against oxidative DNA damage and during ageing is well described	topic_bc
74531	1	354718	6	NULL	NULL	0	NULL	ATM gene	GP	mutation of	increases					breast cancer	MedicalFinding	risk of;; developing			NULL		0	NULL	NULL	NULL	NULL	NULL	Researchers have found that having a mutation in one copy of the ATM gene in each cell (particularly in people who have at least one family member with ataxia-telangiectasia) is associated with an increased risk of developing breast cancer	topic_bc
74532	1	354719	6	NULL	NULL	0	NULL	p53	GP		is encoded by					TP53 gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	p53 (also known as protein 53 or tumor protein 53), is a tumor suppressor protein that in humans is encoded by the TP53 gene	topic_bc
74533	2	354719	6	NULL	NULL	0	NULL	p53	GP		is a type of					tumor suppressor protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	p53 (also known as protein 53 or tumor protein 53), is a tumor suppressor protein that in humans is encoded by the TP53 gene	topic_bc
74534	3	354719	6	NULL	NULL	0	NULL	p53	GP		is a type of					protein 53	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	p53 (also known as protein 53 or tumor protein 53), is a tumor suppressor protein that in humans is encoded by the TP53 gene	topic_bc
74535	4	354719	6	NULL	NULL	0	NULL	p53	GP		is a type of					tumor protein 53	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	p53 (also known as protein 53 or tumor protein 53), is a tumor suppressor protein that in humans is encoded by the TP53 gene	topic_bc
74536	1	354720	6	NULL	NULL	0	NULL	p53	GP	mutant	is associated with					breast cancer	MedicalFinding	aggresive			NULL		0	NULL	NULL	NULL	NULL	NULL	In breast cancer, p53 mutation is associated with more aggressive disease and worse overall survival	topic_bc
74537	2	354720	6	NULL	NULL	NULL	NULL	p53	GP	mutant	is associated with					worse overall survival	Process				NULL	breast cancer	NULL	NULL	NULL	NULL	NULL	NULL	In breast cancer, p53 mutation is associated with more aggressive disease and worse overall survival	topic_bc
74538	1	354722	6	NULL	NULL	0	NULL	CHEK2	GP	abnormal variant of 	develops					breast cancer	MedicalFinding				NULL	women	0	NULL	NULL	NULL	NULL	NULL	Women who carry an abnormal variant of a gene known as CHEK2 are three times more likely to develop breast cancer than women who do not have	topic_bc
74539	1	354724	6	NULL	NULL	0	NULL	PTEN gene	GP	mutant	leads to					breast cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 50 percent of patients with breast cancer have a mutation in or loss of at least one copy of the PTEN gene	topic_bc
74540	1	354725	6	NULL	NULL	0	NULL	CDH1 gene	GP		encodes					Cadherin-1	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Cadherin-1 is a protein that in humans is encoded by the CDH1 gene.	topic_bc
74541	1	354726	6	NULL	NULL	0	NULL	E-cadherin gene	GP	mutation of	increases					breast cancer	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	a mutation of the E-cadherin gene, puts the person at a 40% risk of breast cancer	topic_bc
74542	1	354727	6	NULL	NULL	0	NULL	Sixteen-carbon metabolites	Chemical		are toxic to					cellular DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	Sixteen-carbon metabolites are also toxic to cellular DNA. Synthetic xenoestrogens apparently block the 2-carbon pathway and promote 16-carbon metabolism	topic_bc
73761	1	354728	5	NULL	NULL	0	NULL	cerebellum	OrganismPart		plays a role in		may			pain perception	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The roles of the cerebellum in pain perception, attention deficit disorder, autism, dementia, and schizophrenia are discussed. 	topic_sch
73762	2	354728	5	NULL	NULL	0	NULL	cerebellum	OrganismPart		plays a role in		may			attention deficit disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The roles of the cerebellum in pain perception, attention deficit disorder, autism, dementia, and schizophrenia are discussed. 	topic_sch
73763	3	354728	5	NULL	NULL	0	NULL	cerebellum	OrganismPart		plays a role in		may			autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The roles of the cerebellum in pain perception, attention deficit disorder, autism, dementia, and schizophrenia are discussed. 	topic_sch
73764	4	354728	5	NULL	NULL	0	NULL	cerebellum	OrganismPart		plays a role in		may			dementia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The roles of the cerebellum in pain perception, attention deficit disorder, autism, dementia, and schizophrenia are discussed. 	topic_sch
73765	5	354728	5	NULL	NULL	0	NULL	cerebellum	OrganismPart		plays a role in		may			schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The roles of the cerebellum in pain perception, attention deficit disorder, autism, dementia, and schizophrenia are discussed. 	topic_sch
74543	1	354729	6	NULL	NULL	0	NULL	Obesity	PhysicalPhenomenon		risks					breast cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity is a well-known risk factor for breast cancer after menopause	topic_bc
73766	1	354730	5	NULL	NULL	0	NULL	DNA viruses	Organism		infects					mother	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Maternal infection during pregnancy with a wide range of RNA and DNA viruses is associated with increased risk for schizophrenia and autism in their offspring.	topic_sch
73767	2	354730	5	NULL	NULL	0	NULL	statement 1	Process		occurs during					pregnancy	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Maternal infection during pregnancy with a wide range of RNA and DNA viruses is associated with increased risk for schizophrenia and autism in their offspring.	topic_sch
73768	3	354730	5	NULL	NULL	0	NULL	RNA viruses	Organism		infects					mother	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Maternal infection during pregnancy with a wide range of RNA and DNA viruses is associated with increased risk for schizophrenia and autism in their offspring.	topic_sch
73769	4	354730	5	NULL	NULL	0	NULL	statement 3	Process		occurs during					pregnancy	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Maternal infection during pregnancy with a wide range of RNA and DNA viruses is associated with increased risk for schizophrenia and autism in their offspring.	topic_sch
73770	5	354730	5	NULL	NULL	0	NULL	statement 2	Process		is associated with					schizophrenia	MedicalFinding	increased risk for			NULL	offspring	0	NULL	NULL	NULL	NULL	NULL	Maternal infection during pregnancy with a wide range of RNA and DNA viruses is associated with increased risk for schizophrenia and autism in their offspring.	topic_sch
73771	6	354730	5	NULL	NULL	0	NULL	statement 2	Process		is associated with					autism	MedicalFinding	increased risk for			NULL	offspring	0	NULL	NULL	NULL	NULL	NULL	Maternal infection during pregnancy with a wide range of RNA and DNA viruses is associated with increased risk for schizophrenia and autism in their offspring.	topic_sch
73772	7	354730	5	NULL	NULL	0	NULL	statement 4	Process		is associated with					schizophrenia	MedicalFinding	increased risk for			NULL	offspring	0	NULL	NULL	NULL	NULL	NULL	Maternal infection during pregnancy with a wide range of RNA and DNA viruses is associated with increased risk for schizophrenia and autism in their offspring.	topic_sch
73773	8	354730	5	NULL	NULL	0	NULL	statement 4	Process		is associated with					autism	MedicalFinding	increased risk for			NULL	offspring	0	NULL	NULL	NULL	NULL	NULL	Maternal infection during pregnancy with a wide range of RNA and DNA viruses is associated with increased risk for schizophrenia and autism in their offspring.	topic_sch
73778	1	354731	5	NULL	NULL	0	NULL	ASD patients	GroupOfPeople		shows					schizophrenia spectrum traits	MedicalFinding				NULL	adolescence	0	NULL	NULL	NULL	NULL	NULL	These findings indicate that patients diagnosed with an ASD show schizophrenia spectrum traits in adolescence. 	topic_sch
73779	1	354732	5	NULL	NULL	0	NULL	birth weight	PhysicalPhenomenon	low 	increases					schizophrenia	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	Both low (OR 2.5; 95% CI 1.2-5.1) and high birth weight (OR 2.4; 95% CI 1.1-4.9) increased the risk of later schizophrenia. 	topic_sch
73780	2	354732	5	NULL	NULL	0	NULL	birth weight	PhysicalPhenomenon	high	increases					schizophrenia	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	Both low (OR 2.5; 95% CI 1.2-5.1) and high birth weight (OR 2.4; 95% CI 1.1-4.9) increased the risk of later schizophrenia. 	topic_sch
73781	1	354733	5	NULL	NULL	NULL	NULL	babies	Organism	short	is at risk of		elevated			schizophrenia	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition, short (OR 2.6; 95% CI 1.1-5.9) and long babies had an elevated risk of schizophrenia as adults (OR 1.8; 95% CI 1.0-3.5).	topic_sch
73782	2	354733	5	NULL	NULL	NULL	NULL	babies	Organism	long	is at risk of		elevated			schizophrenia	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition, short (OR 2.6; 95% CI 1.1-5.9) and long babies had an elevated risk of schizophrenia as adults (OR 1.8; 95% CI 1.0-3.5).	topic_sch
73783	1	354734	5	NULL	NULL	0	NULL	potassium channel genes	GP		is a type of					candidate genes	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies have reported that some potassium channel genes might be candidate genes for susceptibility to schizophrenia.	topic_sch
73784	2	354734	5	NULL	NULL	0	NULL	statement 1	GP		is susceptible to					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies have reported that some potassium channel genes might be candidate genes for susceptibility to schizophrenia.	topic_sch
73785	1	354735	5	NULL	NULL	0	NULL	KCNH1	GP		is a type of					potassium channel gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study, we chose three potassium channel genes, KCNH1, KCNJ10, KCNN3 to investigate the role of potassium channels in schizophrenia by genotyping 23 SNPs (9 in KCNH1, 5 in KCNJ10 and 9 in KCNN3) in a Han Chinese sample consisting of 893 schizophrenia patients and 611 healthy controls. No significant difference in allelic or genotypic frequency was revealed between schizophrenia patients and healthy individuals. Nor was a significant difference in haplotypic distribution detected. MDR analysis revealed no gene-gene interaction within the three potassium channel genes. Our study suggests that the 23 SNPs within the three potassium genes we examined do not play a major role in schizophrenia in the Han Chinese population.	topic_sch
73786	2	354735	5	NULL	NULL	0	NULL	KCNJ10	GP		is a type of					potassium channel gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study, we chose three potassium channel genes, KCNH1, KCNJ10, KCNN3 to investigate the role of potassium channels in schizophrenia by genotyping 23 SNPs (9 in KCNH1, 5 in KCNJ10 and 9 in KCNN3) in a Han Chinese sample consisting of 893 schizophrenia patients and 611 healthy controls. No significant difference in allelic or genotypic frequency was revealed between schizophrenia patients and healthy individuals. Nor was a significant difference in haplotypic distribution detected. MDR analysis revealed no gene-gene interaction within the three potassium channel genes. Our study suggests that the 23 SNPs within the three potassium genes we examined do not play a major role in schizophrenia in the Han Chinese population.	topic_sch
73787	3	354735	5	NULL	NULL	0	NULL	KCNN3	GP		is a type of					potassium channel gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study, we chose three potassium channel genes, KCNH1, KCNJ10, KCNN3 to investigate the role of potassium channels in schizophrenia by genotyping 23 SNPs (9 in KCNH1, 5 in KCNJ10 and 9 in KCNN3) in a Han Chinese sample consisting of 893 schizophrenia patients and 611 healthy controls. No significant difference in allelic or genotypic frequency was revealed between schizophrenia patients and healthy individuals. Nor was a significant difference in haplotypic distribution detected. MDR analysis revealed no gene-gene interaction within the three potassium channel genes. Our study suggests that the 23 SNPs within the three potassium genes we examined do not play a major role in schizophrenia in the Han Chinese population.	topic_sch
73788	4	354735	5	NULL	NULL	0	NULL	KCNH1 SNPs	GP		does not play a role in		major			schizophrenia	MedicalFinding				NULL	Han Chinese population	0	NULL	NULL	NULL	NULL	NULL	In the present study, we chose three potassium channel genes, KCNH1, KCNJ10, KCNN3 to investigate the role of potassium channels in schizophrenia by genotyping 23 SNPs (9 in KCNH1, 5 in KCNJ10 and 9 in KCNN3) in a Han Chinese sample consisting of 893 schizophrenia patients and 611 healthy controls. No significant difference in allelic or genotypic frequency was revealed between schizophrenia patients and healthy individuals. Nor was a significant difference in haplotypic distribution detected. MDR analysis revealed no gene-gene interaction within the three potassium channel genes. Our study suggests that the 23 SNPs within the three potassium genes we examined do not play a major role in schizophrenia in the Han Chinese population.	topic_sch
73789	5	354735	5	NULL	NULL	0	NULL	KCNJ10 SNPs	GP		does not play a role in		major			schizophrenia	MedicalFinding				NULL	Han Chinese population	0	NULL	NULL	NULL	NULL	NULL	In the present study, we chose three potassium channel genes, KCNH1, KCNJ10, KCNN3 to investigate the role of potassium channels in schizophrenia by genotyping 23 SNPs (9 in KCNH1, 5 in KCNJ10 and 9 in KCNN3) in a Han Chinese sample consisting of 893 schizophrenia patients and 611 healthy controls. No significant difference in allelic or genotypic frequency was revealed between schizophrenia patients and healthy individuals. Nor was a significant difference in haplotypic distribution detected. MDR analysis revealed no gene-gene interaction within the three potassium channel genes. Our study suggests that the 23 SNPs within the three potassium genes we examined do not play a major role in schizophrenia in the Han Chinese population.	topic_sch
73790	6	354735	5	NULL	NULL	0	NULL	KCNN3 SNPs	GP		does not play a role in		major			schizophrenia	MedicalFinding				NULL	Han Chinese population	0	NULL	NULL	NULL	NULL	NULL	In the present study, we chose three potassium channel genes, KCNH1, KCNJ10, KCNN3 to investigate the role of potassium channels in schizophrenia by genotyping 23 SNPs (9 in KCNH1, 5 in KCNJ10 and 9 in KCNN3) in a Han Chinese sample consisting of 893 schizophrenia patients and 611 healthy controls. No significant difference in allelic or genotypic frequency was revealed between schizophrenia patients and healthy individuals. Nor was a significant difference in haplotypic distribution detected. MDR analysis revealed no gene-gene interaction within the three potassium channel genes. Our study suggests that the 23 SNPs within the three potassium genes we examined do not play a major role in schizophrenia in the Han Chinese population.	topic_sch
73791	1	354736	5	NULL	NULL	0	NULL	DAO	GP		is					D-amino acid oxidase	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	D-amino acid oxidase (DAO), an enzyme that degrades D-serine, has been suggested as a susceptibility factor for schizophrenia.	topic_sch
73792	2	354736	5	NULL	NULL	0	NULL	DAO	GP		is a type of					enzyme	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	D-amino acid oxidase (DAO), an enzyme that degrades D-serine, has been suggested as a susceptibility factor for schizophrenia.	topic_sch
73793	3	354736	5	NULL	NULL	0	NULL	DAO	GP		degrades					D-serine	AminoAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	D-amino acid oxidase (DAO), an enzyme that degrades D-serine, has been suggested as a susceptibility factor for schizophrenia.	topic_sch
73794	4	354736	5	NULL	NULL	0	NULL	DAO	GP		is a susceptibility factor for					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	D-amino acid oxidase (DAO), an enzyme that degrades D-serine, has been suggested as a susceptibility factor for schizophrenia.	topic_sch
73795	1	354737	5	NULL	NULL	0	NULL	delusions			enhance					self-esteem					NULL		0	NULL	NULL	NULL	NULL	NULL	Although these findings do not support the hypothesis that delusions serve to enhance self-esteem, they underline the relevance of low self-esteem in patients with persecutory delusions and point to the necessity of enhancing self-esteem in therapy.	topic_sch
73796	1	354738	5	NULL	NULL	0	NULL	subjective experiences	Process		is associated with					schizophrenia	MedicalFinding	positive symptomatology in			NULL		0	NULL	NULL	NULL	NULL	NULL	The results of our study suggest that subjective experiences are significantly associated with positive symptomatology in schizophrenia, suggesting that they may share a common underlying neural basis.	topic_sch
73797	1	354739	5	NULL	NULL	0	NULL	estrogen	GP	oral	reduce		might			schizophrenia	MedicalFinding	symptom severity in			NULL		0	NULL	NULL	NULL	NULL	NULL	Emerging evidence from clinical trials suggests that oral estrogen and intranasal oxytocin might reduce symptom severity in schizophrenia. 	topic_sch
73798	2	354739	5	NULL	NULL	0	NULL	oxytocin	GP	intranasal	reduce		might			schizophrenia	MedicalFinding	symptom severity in			NULL		0	NULL	NULL	NULL	NULL	NULL	Emerging evidence from clinical trials suggests that oral estrogen and intranasal oxytocin might reduce symptom severity in schizophrenia. 	topic_sch
73799	1	354740	5	NULL	NULL	0	NULL	environmental stressors	PhysicalPhenomenon		exerts					brain	OrganismPart	major impact on;;development of			NULL		0	NULL	NULL	NULL	NULL	NULL	Environmental stressors during gestation can exert a major impact on brain development and thereby contribute to the pathogenesis of neuropsychiatric illnesses, such as depression and psychotic disorders including schizophrenia.	topic_sch
73800	2	354740	5	NULL	NULL	0	NULL	statement 1	Process		occurs during					gestation	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Environmental stressors during gestation can exert a major impact on brain development and thereby contribute to the pathogenesis of neuropsychiatric illnesses, such as depression and psychotic disorders including schizophrenia.	topic_sch
73801	3	354740	5	NULL	NULL	0	NULL	statement 1	Process		contribute to					depression	MedicalFinding	pathogenesis of			NULL		0	NULL	NULL	NULL	NULL	NULL	Environmental stressors during gestation can exert a major impact on brain development and thereby contribute to the pathogenesis of neuropsychiatric illnesses, such as depression and psychotic disorders including schizophrenia.	topic_sch
73802	4	354740	5	NULL	NULL	0	NULL	depression	MedicalFinding		is a type of					neuropsychiatric illness	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Environmental stressors during gestation can exert a major impact on brain development and thereby contribute to the pathogenesis of neuropsychiatric illnesses, such as depression and psychotic disorders including schizophrenia.	topic_sch
73803	5	354740	5	NULL	NULL	0	NULL	statement 1	Process		contribute to					schizophrenia	MedicalFinding	pathogenesis of			NULL		0	NULL	NULL	NULL	NULL	NULL	Environmental stressors during gestation can exert a major impact on brain development and thereby contribute to the pathogenesis of neuropsychiatric illnesses, such as depression and psychotic disorders including schizophrenia.	topic_sch
73804	6	354740	5	NULL	NULL	0	NULL	schizophrenia	MedicalFinding		is a type of					psychotic disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Environmental stressors during gestation can exert a major impact on brain development and thereby contribute to the pathogenesis of neuropsychiatric illnesses, such as depression and psychotic disorders including schizophrenia.	topic_sch
73805	1	354741	5	NULL	NULL	0	NULL	sildenafil 	Chemical		is adjunctive treatment strategy for		potential			schizophrenia	MedicalFinding	treatment of;;negative symptoms of			NULL		0	NULL	NULL	NULL	NULL	NULL	The present study indicates sildenafil as a potential adjunctive treatment strategy for treatment of negative symptoms of schizophrenia	topic_sch
73806	1	354742	5	NULL	NULL	0	NULL	mGluR2/3 agonist	Chemical		is effective in					anxiety	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical trials have demonstrated positive proof of efficacy of dual metabotropic glutamate receptor 2/3 (mGluR2/3) agonists in both anxiety and schizophrenia.	topic_sch
73807	2	354742	5	NULL	NULL	0	NULL	mGluR2/3 agonist	Chemical		is effective in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical trials have demonstrated positive proof of efficacy of dual metabotropic glutamate receptor 2/3 (mGluR2/3) agonists in both anxiety and schizophrenia.	topic_sch
73808	3	354742	5	NULL	NULL	0	NULL	mGluR2/3	GP		is					metabotropic glutamate receptor 2/3	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical trials have demonstrated positive proof of efficacy of dual metabotropic glutamate receptor 2/3 (mGluR2/3) agonists in both anxiety and schizophrenia.	topic_sch
73809	1	354743	5	NULL	NULL	0	NULL	MONW individuals	GroupOfPeople		is present in					non-diabetic schizophrenia patients	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	The MONW individuals in non-diabetic schizophrenia patients seem to have an unfavorable metabolic profile and significant atherogenecity. 	topic_sch
73810	2	354743	5	NULL	NULL	NULL	NULL	statement 1	GroupOfPeople		possess					unfavorable metabolic profile	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	The MONW individuals in non-diabetic schizophrenia patients seem to have an unfavorable metabolic profile and significant atherogenecity. 	topic_sch
73811	3	354743	5	NULL	NULL	0	NULL	statement 1	GroupOfPeople		possess					atherogenecity	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The MONW individuals in non-diabetic schizophrenia patients seem to have an unfavorable metabolic profile and significant atherogenecity. 	topic_sch
73812	1	354744	5	NULL	NULL	NULL	NULL	negative symptoms	MedicalFinding		is associated with					mental state concept	MentalProcess	lack of			NULL	schizophrenic patients	NULL	NULL	NULL	NULL	NULL	NULL	In schizophrenic patients, negative symptoms were associated with a lack of a mental state concept, while positive symptoms like delusions were associated with 'overmentalizing', supporting respective etiological concepts of delusions	topic_sch
73813	2	354744	5	NULL	NULL	0	NULL	delusion	MedicalFinding		is a type of					positive symptom	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In schizophrenic patients, negative symptoms were associated with a lack of a mental state concept, while positive symptoms like delusions were associated with 'overmentalizing', supporting respective etiological concepts of delusions	topic_sch
73814	3	354744	5	NULL	NULL	0	NULL	delusion	MedicalFinding		is associated with					overmentalizing	MedicalFinding				NULL	schizophrenic patients	0	NULL	NULL	NULL	NULL	NULL	In schizophrenic patients, negative symptoms were associated with a lack of a mental state concept, while positive symptoms like delusions were associated with 'overmentalizing', supporting respective etiological concepts of delusions	topic_sch
73815	1	354745	5	NULL	NULL	0	NULL	ketamine	Chemical		is a type of					noncompetitive N-methyl-D-aspartate antagonist	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Given the evidence that ketamine, a noncompetitive N-methyl-D-aspartate antagonist reproduces symptoms of schizophrenia, we sought to determine whether the rubber-hand illusion is augmented by ketamine.	topic_sch
73816	2	354745	5	NULL	NULL	0	NULL	ketamine	Chemical		reproduces					schizophrenia	MedicalFinding	symptoms of			NULL		0	NULL	NULL	NULL	NULL	NULL	Given the evidence that ketamine, a noncompetitive N-methyl-D-aspartate antagonist reproduces symptoms of schizophrenia, we sought to determine whether the rubber-hand illusion is augmented by ketamine.	topic_sch
73817	3	354745	5	NULL	NULL	0	NULL	rubber-hand illusion	Process		is augmented by		may be			ketamine	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Given the evidence that ketamine, a noncompetitive N-methyl-D-aspartate antagonist reproduces symptoms of schizophrenia, we sought to determine whether the rubber-hand illusion is augmented by ketamine.	topic_sch
73818	1	354747	5	NULL	NULL	0	NULL	serotonin	Chemical		plays a role in					depression	MedicalFinding	etiology of			NULL		0	NULL	NULL	NULL	NULL	NULL	The profusion of 5-HT receptors should eventually allow a better understanding of the different and complex processes in which serotonin is involved. Its role is expected in the ethiology of several diseases, including depression, schizophrenia, anxiety and panic disorders, migraine, hypertension, pulmonary hypertension, eating disorders, vomiting and irritable bowel syndromes	topic_sch
73819	2	354747	5	NULL	NULL	0	NULL	serotonin	Chemical		plays a role in					schizophrenia	MedicalFinding	etiology of			NULL		0	NULL	NULL	NULL	NULL	NULL	The profusion of 5-HT receptors should eventually allow a better understanding of the different and complex processes in which serotonin is involved. Its role is expected in the ethiology of several diseases, including depression, schizophrenia, anxiety and panic disorders, migraine, hypertension, pulmonary hypertension, eating disorders, vomiting and irritable bowel syndromes	topic_sch
73820	3	354747	5	NULL	NULL	0	NULL	serotonin	Chemical		plays a role in					anxiety and panic disorders	MedicalFinding	etiology of			NULL		0	NULL	NULL	NULL	NULL	NULL	The profusion of 5-HT receptors should eventually allow a better understanding of the different and complex processes in which serotonin is involved. Its role is expected in the ethiology of several diseases, including depression, schizophrenia, anxiety and panic disorders, migraine, hypertension, pulmonary hypertension, eating disorders, vomiting and irritable bowel syndromes	topic_sch
73821	4	354747	5	NULL	NULL	0	NULL	serotonin	Chemical		plays a role in					migraine	MedicalFinding	etiology of			NULL		0	NULL	NULL	NULL	NULL	NULL	The profusion of 5-HT receptors should eventually allow a better understanding of the different and complex processes in which serotonin is involved. Its role is expected in the ethiology of several diseases, including depression, schizophrenia, anxiety and panic disorders, migraine, hypertension, pulmonary hypertension, eating disorders, vomiting and irritable bowel syndromes	topic_sch
73822	5	354747	5	NULL	NULL	0	NULL	serotonin	Chemical		plays a role in					hypertension	MedicalFinding	etiology of			NULL		0	NULL	NULL	NULL	NULL	NULL	The profusion of 5-HT receptors should eventually allow a better understanding of the different and complex processes in which serotonin is involved. Its role is expected in the ethiology of several diseases, including depression, schizophrenia, anxiety and panic disorders, migraine, hypertension, pulmonary hypertension, eating disorders, vomiting and irritable bowel syndromes	topic_sch
73823	6	354747	5	NULL	NULL	0	NULL	serotonin	Chemical		plays a role in					pulmonary hypertension	MedicalFinding	etiology of			NULL		0	NULL	NULL	NULL	NULL	NULL	The profusion of 5-HT receptors should eventually allow a better understanding of the different and complex processes in which serotonin is involved. Its role is expected in the ethiology of several diseases, including depression, schizophrenia, anxiety and panic disorders, migraine, hypertension, pulmonary hypertension, eating disorders, vomiting and irritable bowel syndromes	topic_sch
73824	7	354747	5	NULL	NULL	0	NULL	serotonin	Chemical		plays a role in					eating disorders	MedicalFinding	etiology of			NULL		0	NULL	NULL	NULL	NULL	NULL	The profusion of 5-HT receptors should eventually allow a better understanding of the different and complex processes in which serotonin is involved. Its role is expected in the ethiology of several diseases, including depression, schizophrenia, anxiety and panic disorders, migraine, hypertension, pulmonary hypertension, eating disorders, vomiting and irritable bowel syndromes	topic_sch
73825	8	354747	5	NULL	NULL	0	NULL	serotonin	Chemical		plays a role in					vomiting and irritable bowel syndromes	MedicalFinding	etiology of			NULL		0	NULL	NULL	NULL	NULL	NULL	The profusion of 5-HT receptors should eventually allow a better understanding of the different and complex processes in which serotonin is involved. Its role is expected in the ethiology of several diseases, including depression, schizophrenia, anxiety and panic disorders, migraine, hypertension, pulmonary hypertension, eating disorders, vomiting and irritable bowel syndromes	topic_sch
73826	1	354748	5	NULL	NULL	0	NULL	CB1 receptor	GP	alternation of;;function of	implicated in					depression	MedicalFinding				NULL	human	0	NULL	NULL	NULL	NULL	NULL	Alternation of CB1 receptor function has been implicated in a number of human diseases such as depression, schizophrenia, and obesity (4-6). 	topic_sch
73827	2	354748	5	NULL	NULL	0	NULL	CB1 receptor	GP	alternation of;;function of	implicated in					schizophrenia	MedicalFinding				NULL	human	0	NULL	NULL	NULL	NULL	NULL	Alternation of CB1 receptor function has been implicated in a number of human diseases such as depression, schizophrenia, and obesity (4-6). 	topic_sch
73828	3	354748	5	NULL	NULL	0	NULL	CB1 receptor	GP	alternation of;;function of	implicated in					obesity	MedicalFinding				NULL	human	0	NULL	NULL	NULL	NULL	NULL	Alternation of CB1 receptor function has been implicated in a number of human diseases such as depression, schizophrenia, and obesity (4-6). 	topic_sch
73829	1	354749	5	NULL	NULL	0	NULL	phenotypic defects	PhysicalPhenomenon		overlap		partly			schizophrenia	MedicalFinding	defects of			NULL	mice	0	NULL	NULL	NULL	NULL	NULL	In mice, the deletion of the LPA1 receptor causes some phenotypic defects partly overlapping with those found in schizophrenia.	topic_sch
73830	2	354749	5	NULL	NULL	NULL	NULL	LPA1 receptor	GP	deletion of	causes					statement 1	Process				NULL	mice	NULL	NULL	NULL	NULL	NULL	NULL	In mice, the deletion of the LPA1 receptor causes some phenotypic defects partly overlapping with those found in schizophrenia.	topic_sch
73831	1	354750	5	NULL	NULL	0	NULL	CaMKII	GP		plays a role in		important			neurons	Cell	maturation of			NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, in LPA1 KO mice the α/β isoform ratio of CaMKII, which plays a key role in neuronal maturation during development, was markedly decreased, as found previously in schizophrenia patients.	topic_sch
73832	2	354750	5	NULL	NULL	0	NULL	statement 1	Process		occurs during					development	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, in LPA1 KO mice the α/β isoform ratio of CaMKII, which plays a key role in neuronal maturation during development, was markedly decreased, as found previously in schizophrenia patients.	topic_sch
73833	3	354750	5	NULL	NULL	0	NULL	CaMKII	GP	isoform ratio of	is decreased in		markedly			LPA1 KO mice	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, in LPA1 KO mice the α/β isoform ratio of CaMKII, which plays a key role in neuronal maturation during development, was markedly decreased, as found previously in schizophrenia patients.	topic_sch
73834	4	354750	5	NULL	NULL	0	NULL	CaMKII	GP	isoform ratio of	is decreased in		markedly			schizophrenia patients	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, in LPA1 KO mice the α/β isoform ratio of CaMKII, which plays a key role in neuronal maturation during development, was markedly decreased, as found previously in schizophrenia patients.	topic_sch
73835	1	354751	5	NULL	NULL	NULL	NULL	neurodevelopment disorder	MedicalFinding	primary	affect					cerebral cortex	OrganismPart	normal			NULL	schizophrenia	NULL	NULL	NULL	NULL	NULL	NULL	These findings support a primary neurodevelopment disorder affecting the normal cerebral cortex development in schizophrenia.	topic_sch
73836	1	354752	5	NULL	NULL	0	NULL	relatives of schizophrenia patients	GroupOfPeople		demonstrate					prefrontal cortex	OrganismPart	abnormalities in;;activation of			NULL		0	NULL	NULL	NULL	NULL	NULL	Relatives of schizophrenia patients demonstrate abnormalities in prefrontal cortical activation during executive processing as measured by functional neuroimaging, albeit not consistently. 	topic_sch
73837	2	354752	5	NULL	NULL	0	NULL	statement 1	Process		occurs during					executive processing	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Relatives of schizophrenia patients demonstrate abnormalities in prefrontal cortical activation during executive processing as measured by functional neuroimaging, albeit not consistently. 	topic_sch
73838	1	354753	5	NULL	NULL	0	NULL	DUI	Time	prolonged	represents					prognostic factor		negative			NULL		0	NULL	NULL	NULL	NULL	NULL	A significant body of evidence shows that a prolonged DUI represents a negative prognostic factor particularly in schizophrenia.	topic_sch
73839	2	354753	5	NULL	NULL	0	NULL	statement 1	Process		occurs in		particularly			schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	A significant body of evidence shows that a prolonged DUI represents a negative prognostic factor particularly in schizophrenia.	topic_sch
73840	1	354754	5	NULL	NULL	0	NULL	Schizophrenic patients	GroupOfPeople		experience					HPA axis	OrganismPart	hyper function of			NULL		0	NULL	NULL	NULL	NULL	NULL	In summary, the evidence suggests people with schizophrenia can experience both hyper- and hypo-function of the HPA axis. 	topic_sch
73841	2	354754	5	NULL	NULL	0	NULL	Schizophrenic patients	GroupOfPeople		experience					HPA axis	OrganismPart	hypo function of			NULL		0	NULL	NULL	NULL	NULL	NULL	In summary, the evidence suggests people with schizophrenia can experience both hyper- and hypo-function of the HPA axis. 	topic_sch
73842	1	354755	5	NULL	NULL	NULL	NULL	Schizophrenic patients	GroupOfPeople		suffer					mortality		premature 			NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is likely that this contributes to the pattern of poor physical health and premature mortality suffered by people with schizophrenia, in particular the high rates of cardiovascular and metabolic disturbance.	topic_sch
73843	2	354755	5	NULL	NULL	0	NULL	Schizophrenic patients	GroupOfPeople		suffer					physical health	PhysicalPhenomenon	poor			NULL		0	NULL	NULL	NULL	NULL	NULL	It is likely that this contributes to the pattern of poor physical health and premature mortality suffered by people with schizophrenia, in particular the high rates of cardiovascular and metabolic disturbance.	topic_sch
73844	3	354755	5	NULL	NULL	0	NULL	Schizophrenic patients	GroupOfPeople		suffer					cardiovascular disturbance	MedicalFinding	high rates of			NULL		0	NULL	NULL	NULL	NULL	NULL	It is likely that this contributes to the pattern of poor physical health and premature mortality suffered by people with schizophrenia, in particular the high rates of cardiovascular and metabolic disturbance.	topic_sch
73845	4	354755	5	NULL	NULL	0	NULL	Schizophrenic patients	GroupOfPeople		suffer					metabolic disturbance	MedicalFinding	high rates of			NULL		0	NULL	NULL	NULL	NULL	NULL	It is likely that this contributes to the pattern of poor physical health and premature mortality suffered by people with schizophrenia, in particular the high rates of cardiovascular and metabolic disturbance.	topic_sch
73846	1	354758	5	NULL	NULL	0	NULL	maternal schizophrenia	MedicalFinding		is predictive to					postpartum psychosis	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	After adjusting for age, parity, unhealthy behaviors, length of antipsychotic treatment, and maternal-fetal attachment, maternal schizophrenia remains predictive to prematurity and postpartum psychosis.	topic_sch
73847	1	354759	5	NULL	NULL	0	NULL	Quetiapine	Chemical		is a type of					atypical antipsychotic agent	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Quetiapine is an atypical antipsychotic agent increasingly used to treat schizophrenia and bipolar disorder in pediatric patients.	topic_sch
73848	2	354759	5	NULL	NULL	0	NULL	Quetiapine	Chemical		treats					schizophrenia	MedicalFinding				NULL	pediatric patients	0	NULL	NULL	NULL	NULL	NULL	Quetiapine is an atypical antipsychotic agent increasingly used to treat schizophrenia and bipolar disorder in pediatric patients.	topic_sch
73849	3	354759	5	NULL	NULL	0	NULL	Quetiapine	Chemical		treats					bipolar disorder	MedicalFinding				NULL	pediatric patients	0	NULL	NULL	NULL	NULL	NULL	Quetiapine is an atypical antipsychotic agent increasingly used to treat schizophrenia and bipolar disorder in pediatric patients.	topic_sch
73850	1	354760	5	NULL	NULL	0	NULL	galantamine	Chemical		is an inhibitor of		weak			acetylcholine esterase	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical studies show that galantamine, a weak acetylcholine (ACh) esterase inhibitor and allosteric potentiator of nicotinic ACh receptors (nAChRs), improves negative and cognitive symptoms in schizophrenia, while donepezil, a potent ACh esterase inhibitor, does not. 	topic_sch
73851	2	354760	5	NULL	NULL	0	NULL	ACh	Chemical		is					acetylcholine	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical studies show that galantamine, a weak acetylcholine (ACh) esterase inhibitor and allosteric potentiator of nicotinic ACh receptors (nAChRs), improves negative and cognitive symptoms in schizophrenia, while donepezil, a potent ACh esterase inhibitor, does not. 	topic_sch
73852	3	354760	5	NULL	NULL	0	NULL	galantamine	Chemical		allosteric potentiator of					nAChRs	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical studies show that galantamine, a weak acetylcholine (ACh) esterase inhibitor and allosteric potentiator of nicotinic ACh receptors (nAChRs), improves negative and cognitive symptoms in schizophrenia, while donepezil, a potent ACh esterase inhibitor, does not. 	topic_sch
73853	4	354760	5	NULL	NULL	0	NULL	nAChRs	GP		is					nicotinic ACh receptors	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical studies show that galantamine, a weak acetylcholine (ACh) esterase inhibitor and allosteric potentiator of nicotinic ACh receptors (nAChRs), improves negative and cognitive symptoms in schizophrenia, while donepezil, a potent ACh esterase inhibitor, does not. 	topic_sch
73854	5	354760	5	NULL	NULL	0	NULL	galantamine	Chemical		improves					schizophrenia	MedicalFinding	negative symptoms of			NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical studies show that galantamine, a weak acetylcholine (ACh) esterase inhibitor and allosteric potentiator of nicotinic ACh receptors (nAChRs), improves negative and cognitive symptoms in schizophrenia, while donepezil, a potent ACh esterase inhibitor, does not. 	topic_sch
73855	6	354760	5	NULL	NULL	0	NULL	galantamine	Chemical		improves					schizophrenia	MedicalFinding	cognitive symptoms of			NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical studies show that galantamine, a weak acetylcholine (ACh) esterase inhibitor and allosteric potentiator of nicotinic ACh receptors (nAChRs), improves negative and cognitive symptoms in schizophrenia, while donepezil, a potent ACh esterase inhibitor, does not. 	topic_sch
73856	7	354760	5	NULL	NULL	0	NULL	donepezil	Chemical		is an inhibitor of		potent			ACh esterase	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical studies show that galantamine, a weak acetylcholine (ACh) esterase inhibitor and allosteric potentiator of nicotinic ACh receptors (nAChRs), improves negative and cognitive symptoms in schizophrenia, while donepezil, a potent ACh esterase inhibitor, does not. 	topic_sch
73857	8	354760	5	NULL	NULL	0	NULL	donepezil	Chemical		does not improve					schizophrenia	MedicalFinding	negative symptoms of			NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical studies show that galantamine, a weak acetylcholine (ACh) esterase inhibitor and allosteric potentiator of nicotinic ACh receptors (nAChRs), improves negative and cognitive symptoms in schizophrenia, while donepezil, a potent ACh esterase inhibitor, does not. 	topic_sch
73858	9	354760	5	NULL	NULL	0	NULL	donepezil	Chemical		does not improve					schizophrenia	MedicalFinding	cognitive symptoms of			NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical studies show that galantamine, a weak acetylcholine (ACh) esterase inhibitor and allosteric potentiator of nicotinic ACh receptors (nAChRs), improves negative and cognitive symptoms in schizophrenia, while donepezil, a potent ACh esterase inhibitor, does not. 	topic_sch
73859	1	354761	5	NULL	NULL	0	NULL	QKI gene	GP	human	is a synonym of					quaking homolog, KH domain RNA binding (mouse)	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The human QKI gene, called quaking homolog, KH domain RNA binding (mouse), is a candidate gene for schizophrenia encoding an RNA-binding protein.	topic_sch
73860	2	354761	5	NULL	NULL	0	NULL	QKI gene	GP	human	is a candidate gene for					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The human QKI gene, called quaking homolog, KH domain RNA binding (mouse), is a candidate gene for schizophrenia encoding an RNA-binding protein.	topic_sch
73861	3	354761	5	NULL	NULL	0	NULL	QKI gene	GP		encodes					RNA-binding protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The human QKI gene, called quaking homolog, KH domain RNA binding (mouse), is a candidate gene for schizophrenia encoding an RNA-binding protein.	topic_sch
73862	1	354762	5	NULL	NULL	0	NULL	CHRNA7	GP		is a candidate gene for					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	CHRNA7 has been shown to be a strong candidate gene for schizophrenia and bipolar disorder.	topic_sch
73863	2	354762	5	NULL	NULL	0	NULL	CHRNA7	GP		is a candidate gene for					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	CHRNA7 has been shown to be a strong candidate gene for schizophrenia and bipolar disorder.	topic_sch
73864	1	354763	5	NULL	NULL	0	NULL	CHRNA7	GP		is a candidate gene for		strong			schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	CHRNA7 has been shown to be a strong candidate gene for schizophrenia and bipolar disorder. It is located on chromosome 15q13-q14, which is one of the replicated linkage spots for schizophrenia and bipolar disorder.	topic_sch
73865	2	354763	5	NULL	NULL	0	NULL	CHRNA7	GP		is a candidate gene for		strong			bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	CHRNA7 has been shown to be a strong candidate gene for schizophrenia and bipolar disorder. It is located on chromosome 15q13-q14, which is one of the replicated linkage spots for schizophrenia and bipolar disorder.	topic_sch
73866	3	354763	5	NULL	NULL	0	NULL	CHRNA7	GP		is located on					chromosome 15q13-q14	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	CHRNA7 has been shown to be a strong candidate gene for schizophrenia and bipolar disorder. It is located on chromosome 15q13-q14, which is one of the replicated linkage spots for schizophrenia and bipolar disorder.	topic_sch
73867	4	354763	5	NULL	NULL	0	NULL	chromosome 15q13-q14	Chromosome		is a linkage spot for					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	CHRNA7 has been shown to be a strong candidate gene for schizophrenia and bipolar disorder. It is located on chromosome 15q13-q14, which is one of the replicated linkage spots for schizophrenia and bipolar disorder.	topic_sch
73868	5	354763	5	NULL	NULL	0	NULL	chromosome 15q13-q14	Chromosome		is a linkage spot for					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	CHRNA7 has been shown to be a strong candidate gene for schizophrenia and bipolar disorder. It is located on chromosome 15q13-q14, which is one of the replicated linkage spots for schizophrenia and bipolar disorder.	topic_sch
73869	1	354764	5	NULL	NULL	0	NULL	schizophrenia outpatients	GroupOfPeople	clinically stable	maintains					remission states					NULL		0	NULL	NULL	NULL	NULL	NULL	This study suggested that most clinically stable outpatients with schizophrenia maintain their remission states after being switched to aripiprazole, without serious symptom aggravation and adverse events over a course of 26 weeks.	topic_sch
73870	2	354764	5	NULL	NULL	0	NULL	aripiprazole	Chemical	switching to	leads to					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	This study suggested that most clinically stable outpatients with schizophrenia maintain their remission states after being switched to aripiprazole, without serious symptom aggravation and adverse events over a course of 26 weeks.	topic_sch
73871	1	354765	5	NULL	NULL	0	NULL	Nrg1	GP		is					Neuregulin 1	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Neuregulin 1 (Nrg1), a schizophrenia susceptibility gene, is involved in fundamental aspects of neurodevelopment. 	topic_sch
73872	2	354765	5	NULL	NULL	0	NULL	Neuregulin 1	GP		is a type of					schizophrenia susceptibility gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Neuregulin 1 (Nrg1), a schizophrenia susceptibility gene, is involved in fundamental aspects of neurodevelopment. 	topic_sch
73873	3	354765	5	NULL	NULL	0	NULL	Neuregulin 1	GP		is involved in					neurodevelopment	Process	fundamental aspects of			NULL		0	NULL	NULL	NULL	NULL	NULL	Neuregulin 1 (Nrg1), a schizophrenia susceptibility gene, is involved in fundamental aspects of neurodevelopment. 	topic_sch
73874	1	354768	5	NULL	NULL	0	NULL	CHRM1	GP		is decreased in		selectively			MRDS patients	GroupOfPeople	frontal cortex regions of			NULL		0	NULL	NULL	NULL	NULL	NULL	Having recently shown that CHRM1 levels are decreased selectively in frontal cortex regions of a subpopulation of schizophrenic patients (muscarinic receptor deficit schizophrenia, MRDS) we aimed to compare the protein expression of BACE1 and NRG1 in the agranular frontal cortex Brodmann's area 6 of SCZ subjects with normal levels of CHRM1 (N=19), MRDS (N=20), and age/gender-matched non-psychiatric (healthy) controls (HC; N=20).	topic_sch
73875	2	354768	5	NULL	NULL	0	NULL	MRDS	MedicalFinding		is					muscarinic receptor deficit schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Having recently shown that CHRM1 levels are decreased selectively in frontal cortex regions of a subpopulation of schizophrenic patients (muscarinic receptor deficit schizophrenia, MRDS) we aimed to compare the protein expression of BACE1 and NRG1 in the agranular frontal cortex Brodmann's area 6 of SCZ subjects with normal levels of CHRM1 (N=19), MRDS (N=20), and age/gender-matched non-psychiatric (healthy) controls (HC; N=20).	topic_sch
73876	3	354768	5	NULL	NULL	0	NULL	MRDS	MedicalFinding		is a subpopulation of					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Having recently shown that CHRM1 levels are decreased selectively in frontal cortex regions of a subpopulation of schizophrenic patients (muscarinic receptor deficit schizophrenia, MRDS) we aimed to compare the protein expression of BACE1 and NRG1 in the agranular frontal cortex Brodmann's area 6 of SCZ subjects with normal levels of CHRM1 (N=19), MRDS (N=20), and age/gender-matched non-psychiatric (healthy) controls (HC; N=20).	topic_sch
73877	1	354769	5	NULL	NULL	0	NULL	NRG1	GP	proteolytic processing of 	is impaired in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that the proteolytic processing of NRG1 is impaired in schizophrenia.	topic_sch
73774	1	354770	7	NULL	NULL	0	NULL	Bipolar I disorder	MedicalFinding		is a type of					mood disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar I disorder is a mood disorder that is characterized by at least one manic or mixed episode.	topic_bd
73775	2	354770	7	NULL	NULL	0	NULL	statement 1	Process		characterized by					manic episode	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar I disorder is a mood disorder that is characterized by at least one manic or mixed episode.	topic_bd
73776	3	354770	7	NULL	NULL	0	NULL	statement 1	Process		characterized by					mixed eposode	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar I disorder is a mood disorder that is characterized by at least one manic or mixed episode.	topic_bd
73777	1	354771	7	NULL	NULL	0	NULL	Bipolar II disorder	MedicalFinding		is a type of					bipolar spectrum disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar II disorder is a bipolar spectrum disorder characterized by at least one hypomanic episode and at least one major depressive episode; with this disorder, depressive episodes are more frequent and more intense than manic episodes.	topic_bd
73989	2	354771	7	NULL	NULL	0	NULL	statement 1	Process		characterized by					 hypomanic episode	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar II disorder is a bipolar spectrum disorder characterized by at least one hypomanic episode and at least one major depressive episode; with this disorder, depressive episodes are more frequent and more intense than manic episodes.	topic_bd
73990	3	354771	7	NULL	NULL	NULL	NULL	statement 1	Process		characterized by					major depressive episode	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bipolar II disorder is a bipolar spectrum disorder characterized by at least one hypomanic episode and at least one major depressive episode; with this disorder, depressive episodes are more frequent and more intense than manic episodes.	topic_bd
73991	4	354771	7	NULL	NULL	NULL	NULL	depressive episodes 	MedicalFinding	frequency of	is more than					manic episodes	MedicalFinding	frequency of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bipolar II disorder is a bipolar spectrum disorder characterized by at least one hypomanic episode and at least one major depressive episode; with this disorder, depressive episodes are more frequent and more intense than manic episodes.	topic_bd
73992	5	354771	7	NULL	NULL	0	NULL	depressive episodes 	MedicalFinding		more intense than					manic episodes	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar II disorder is a bipolar spectrum disorder characterized by at least one hypomanic episode and at least one major depressive episode; with this disorder, depressive episodes are more frequent and more intense than manic episodes.	topic_bd
73993	1	354772	7	NULL	NULL	0	NULL	Bipolar disorder	MedicalFinding		is a type of					mental illness	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar disorder is a serious mental illness that is characterized by extreme changes in mood, from mania to depression.	topic_bd
73994	2	354772	7	NULL	NULL	0	NULL	mania	MedicalFinding		changed to					depression	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar disorder is a serious mental illness that is characterized by extreme changes in mood, from mania to depression.	topic_bd
73995	3	354772	7	NULL	NULL	NULL	NULL	statement 1	Process		characterized by					statement 2	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bipolar disorder is a serious mental illness that is characterized by extreme changes in mood, from mania to depression.	topic_bd
73996	1	354773	7	NULL	NULL	0	NULL	Women	GroupOfPeople		have more					mood episode	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Women are also at higher risk for rapid cycling, which means having four or more mood episodes in one year.	topic_bd
74001	1	354774	7	NULL	NULL	0	NULL	 bipolar disorder	MedicalFinding		involves					genetic component	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Experts do believe that bipolar disorder often runs in families, and there is a genetic component to this mood disorder.	topic_bd
73997	1	354775	7	NULL	NULL	0	NULL	bipolar disorder	MedicalFinding	treatment of	more difficult with					alcohol	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Stressful life events -- or alcohol or drug abuse -- can make bipolar disorder more difficult to treat.	topic_bd
73998	2	354775	7	NULL	NULL	NULL	NULL	bipolar disorder	MedicalFinding	treatment of	more difficult with					drug abuse	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Stressful life events -- or alcohol or drug abuse -- can make bipolar disorder more difficult to treat.	topic_bd
73999	1	354776	7	NULL	NULL	0	NULL	bipolar disorder	MedicalFinding		caused by		partly			neurotransmitter	Chemical	underlying problem with the balance of			NULL		0	NULL	NULL	NULL	NULL	NULL	Experts believe bipolar disorder is partly caused by an underlying problem with the balance of brain chemicals called neurotransmitters.	topic_bd
74000	2	354776	7	NULL	NULL	0	NULL	neurotransmitter	Chemical		is a type of					brain chemical	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Experts believe bipolar disorder is partly caused by an underlying problem with the balance of brain chemicals called neurotransmitters.	topic_bd
74002	1	354777	7	NULL	NULL	0	NULL	noradrenaline	Chemical		involved in					brain function	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Three brain chemicals -- noradrenaline (norepinephrine), serotonin, and dopamine -- are involved in both brain and bodily functions. 	topic_bd
74003	2	354777	7	NULL	NULL	0	NULL	serotonin	Chemical		involved in					brain function	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Three brain chemicals -- noradrenaline (norepinephrine), serotonin, and dopamine -- are involved in both brain and bodily functions. 	topic_bd
74004	3	354777	7	NULL	NULL	0	NULL	dopamine	Chemical		involved in					brain function	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Three brain chemicals -- noradrenaline (norepinephrine), serotonin, and dopamine -- are involved in both brain and bodily functions. 	topic_bd
74005	4	354777	7	NULL	NULL	0	NULL	noradrenaline	Chemical		involved in					body function	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Three brain chemicals -- noradrenaline (norepinephrine), serotonin, and dopamine -- are involved in both brain and bodily functions. 	topic_bd
74006	5	354777	7	NULL	NULL	0	NULL	serotonin	Chemical		involved in					body function	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Three brain chemicals -- noradrenaline (norepinephrine), serotonin, and dopamine -- are involved in both brain and bodily functions. 	topic_bd
74007	6	354777	7	NULL	NULL	0	NULL	dopamine	Chemical		involved in					body function	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Three brain chemicals -- noradrenaline (norepinephrine), serotonin, and dopamine -- are involved in both brain and bodily functions. 	topic_bd
74008	7	354777	7	NULL	NULL	0	NULL	 noradrenaline	Chemical		is					norepinephrine	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Three brain chemicals -- noradrenaline (norepinephrine), serotonin, and dopamine -- are involved in both brain and bodily functions. 	topic_bd
74009	8	354777	7	NULL	NULL	0	NULL	noradrenaline	Chemical		is a type of					brain chemical	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Three brain chemicals -- noradrenaline (norepinephrine), serotonin, and dopamine -- are involved in both brain and bodily functions. 	topic_bd
74010	9	354777	7	NULL	NULL	0	NULL	serotonin	Chemical		is a type of					brain chemical	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Three brain chemicals -- noradrenaline (norepinephrine), serotonin, and dopamine -- are involved in both brain and bodily functions. 	topic_bd
74011	10	354777	7	NULL	NULL	0	NULL	dopamine	Chemical		is a type of					brain chemical	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Three brain chemicals -- noradrenaline (norepinephrine), serotonin, and dopamine -- are involved in both brain and bodily functions. 	topic_bd
74012	1	354778	7	NULL	NULL	0	NULL	Noradrenaline	Chemical		linked to					depression	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Noradrenaline and serotonin have been consistently linked to psychiatric mood disorders such as depression and bipolar disorder.	topic_bd
74013	2	354778	7	NULL	NULL	0	NULL	Noradrenaline	Chemical		linked to					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Noradrenaline and serotonin have been consistently linked to psychiatric mood disorders such as depression and bipolar disorder.	topic_bd
74014	3	354778	7	NULL	NULL	0	NULL	serotonin	Chemical		linked to					depression	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Noradrenaline and serotonin have been consistently linked to psychiatric mood disorders such as depression and bipolar disorder.	topic_bd
74015	4	354778	7	NULL	NULL	0	NULL	serotonin	Chemical		linked to					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Noradrenaline and serotonin have been consistently linked to psychiatric mood disorders such as depression and bipolar disorder.	topic_bd
74016	5	354778	7	NULL	NULL	0	NULL	depression	MedicalFinding		is a type of					psychiatric mood disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Noradrenaline and serotonin have been consistently linked to psychiatric mood disorders such as depression and bipolar disorder.	topic_bd
74017	6	354778	7	NULL	NULL	0	NULL	bipolar disorder	MedicalFinding		is a type of					 psychiatric mood disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Noradrenaline and serotonin have been consistently linked to psychiatric mood disorders such as depression and bipolar disorder.	topic_bd
74018	1	354779	7	NULL	NULL	0	NULL	bipolar II	MedicalFinding		diagnosis of		prevalent			bipolar I family	MedicalFinding	relatives in			NULL		0	NULL	NULL	NULL	NULL	NULL	However, among patients with bipolar II, researchers found onlyone relative with bipolar I disorder. They concluded that bipolar II is the most prevalent diagnosis of relatives in both bipolar I and bipolar II families.	topic_bd
74019	2	354779	7	NULL	NULL	0	NULL	 bipolar II	MedicalFinding		diagnosis of		prevalent			bipolar II family	MedicalFinding	relatives in			NULL		0	NULL	NULL	NULL	NULL	NULL	However, among patients with bipolar II, researchers found onlyone relative with bipolar I disorder. They concluded that bipolar II is the most prevalent diagnosis of relatives in both bipolar I and bipolar II families.	topic_bd
74020	1	354780	7	NULL	NULL	0	NULL	 bipolar disorder	MedicalFinding		have 					sleep-wake cycle	Process	genetic predisposition to abnormalities in			NULL		0	NULL	NULL	NULL	NULL	NULL	Some findings show that people with bipolar disorder have a genetic predisposition to sleep-wake cycle abnormalities that may be responsible for triggering the symptoms of depression and mania.	topic_bd
74021	2	354780	7	NULL	NULL	0	NULL	statement 1	Process		responsible for		may be			depression	MedicalFinding	triggering the symptoms of			NULL		0	NULL	NULL	NULL	NULL	NULL	Some findings show that people with bipolar disorder have a genetic predisposition to sleep-wake cycle abnormalities that may be responsible for triggering the symptoms of depression and mania.	topic_bd
74022	3	354780	7	NULL	NULL	NULL	NULL	statement 1	Process		responsible for		may be			mania	MedicalFinding	triggering the symptoms of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Some findings show that people with bipolar disorder have a genetic predisposition to sleep-wake cycle abnormalities that may be responsible for triggering the symptoms of depression and mania.	topic_bd
74023	1	354782	7	NULL	NULL	NULL	NULL	Fish	Organism		help with					 depression	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fish may have earned its reputation as “brain food” because some people eat fish to help with depression, psychosis, attention deficit-hyperactivity disorder (ADHD), Alzheimer’s disease, and other thinking disorders.	topic_bd
74024	2	354782	7	NULL	NULL	NULL	NULL	Fish	Organism		help with					psychosis	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fish may have earned its reputation as “brain food” because some people eat fish to help with depression, psychosis, attention deficit-hyperactivity disorder (ADHD), Alzheimer’s disease, and other thinking disorders.	topic_bd
74025	3	354782	7	NULL	NULL	0	NULL	Fish	Organism		help with					ADHD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Fish may have earned its reputation as “brain food” because some people eat fish to help with depression, psychosis, attention deficit-hyperactivity disorder (ADHD), Alzheimer’s disease, and other thinking disorders.	topic_bd
74026	4	354782	7	NULL	NULL	0	NULL	Fish	Organism		help with					Alzheimer disease	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Fish may have earned its reputation as “brain food” because some people eat fish to help with depression, psychosis, attention deficit-hyperactivity disorder (ADHD), Alzheimer’s disease, and other thinking disorders.	topic_bd
74027	5	354782	7	NULL	NULL	0	NULL	Fish	Organism		help with					thinking disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Fish may have earned its reputation as “brain food” because some people eat fish to help with depression, psychosis, attention deficit-hyperactivity disorder (ADHD), Alzheimer’s disease, and other thinking disorders.	topic_bd
74028	6	354782	7	NULL	NULL	0	NULL	ADHD	MedicalFinding		is					attention deficit-hyperactivity disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Fish may have earned its reputation as “brain food” because some people eat fish to help with depression, psychosis, attention deficit-hyperactivity disorder (ADHD), Alzheimer’s disease, and other thinking disorders.	topic_bd
74029	1	354784	7	NULL	NULL	NULL	NULL	Early onset bipolar disorder	MedicalFinding	symptoms of	 similar to		very			ADHD	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early onset, or juvenile, bipolar disorder has symptoms very similar to ADHD (attention deficit hyperactivity disorder).	topic_bd
74030	2	354784	7	NULL	NULL	NULL	NULL	 juvenile bipolar disorder	MedicalFinding	symptoms of	similar to		very			ADHD	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early onset, or juvenile, bipolar disorder has symptoms very similar to ADHD (attention deficit hyperactivity disorder).	topic_bd
74031	3	354784	7	NULL	NULL	0	NULL	ADHD	MedicalFinding		is					attention deficit hyperactivity disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Early onset, or juvenile, bipolar disorder has symptoms very similar to ADHD (attention deficit hyperactivity disorder).	topic_bd
73878	1	354786	5	NULL	NULL	0	NULL	TGM2	GP		is involved in					schizophrenia	MedicalFinding	dysfunction of;;immune system in			NULL		0	NULL	NULL	NULL	NULL	NULL	TGM2 may be involved in dysfunction of the immune system in schizophrenia.	topic_sch
74544	1	354787	6	NULL	NULL	0	NULL	Papillomatosis	MedicalFinding		is caused by					hyperplasia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Papillomatosis is skin surface elevation caused by hyperplasia	topic_bc
74545	2	354787	6	NULL	NULL	0	NULL	Papillomatosis	MedicalFinding		causes					skin surface	OrganismPart	elevation of			NULL		0	NULL	NULL	NULL	NULL	NULL	Papillomatosis is skin surface elevation caused by hyperplasia	topic_bc
73879	1	354798	5	NULL	NULL	0	NULL	family income	PhysicalPhenomenon		does not affect					autism	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	Family income, education, and lifestyle do not seem to affect the risk of autism.	topic_aut
73880	2	354798	5	NULL	NULL	0	NULL	education	Process		does not affect					autism	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	Family income, education, and lifestyle do not seem to affect the risk of autism.	topic_aut
73881	3	354798	5	NULL	NULL	0	NULL	lifestyle	AbstractConcept		does not affect					autism	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	Family income, education, and lifestyle do not seem to affect the risk of autism.	topic_aut
73882	1	354799	5	NULL	NULL	NULL	NULL	autism	MedicalFinding		is not linked to					MMR vaccine	MedicalProcedure				NULL		NULL	NULL	NULL	NULL	NULL	NULL	The American Academy of Pediatrics and the Center for Disease Control and Prevention report that there is no proven link between autism and the MMR vaccine, or any other vaccine.	topic_aut
73883	1	354800	5	NULL	NULL	0	NULL	Asperger syndrome	MedicalFinding		similar to					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Asperger syndrome (like autism, but with normal language development)	topic_aut
73884	1	354801	5	NULL	NULL	0	NULL	PDD-NOS	MedicalFinding		is					Pervasive developmental disorder - not otherwise specified	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Pervasive developmental disorder - not otherwise specified (PDD-NOS), also called atypical autism.	topic_aut
73885	2	354801	5	NULL	NULL	0	NULL	PDD-NOS	MedicalFinding		is a synonym of					atypical autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Pervasive developmental disorder - not otherwise specified (PDD-NOS), also called atypical autism.	topic_aut
73886	1	354803	5	NULL	NULL	0	NULL	autism	MedicalFinding		is associated with		may be			Fragile X syndrome	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Autism can be associated with other disorders that affect the brain, such as: * Fragile X syndrome * Mental retardation * Tuberous sclerosis	topic_aut
73887	2	354803	5	NULL	NULL	0	NULL	autism	MedicalFinding		is associated with		may be			Mental retardation	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Autism can be associated with other disorders that affect the brain, such as: * Fragile X syndrome * Mental retardation * Tuberous sclerosis	topic_aut
73888	3	354803	5	NULL	NULL	0	NULL	autism	MedicalFinding		is associated with		may be			Mental retardation	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Autism can be associated with other disorders that affect the brain, such as: * Fragile X syndrome * Mental retardation * Tuberous sclerosis	topic_aut
73889	4	354803	5	NULL	NULL	0	NULL	Mental retardation	MedicalFinding		affect					brain	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Autism can be associated with other disorders that affect the brain, such as: * Fragile X syndrome * Mental retardation * Tuberous sclerosis	topic_aut
73890	5	354803	5	NULL	NULL	0	NULL	Fragile X syndrome	MedicalFinding		affect					brain	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Autism can be associated with other disorders that affect the brain, such as: * Fragile X syndrome * Mental retardation * Tuberous sclerosis	topic_aut
73891	6	354803	5	NULL	NULL	0	NULL	Mental retardation	MedicalFinding		affect					brain	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Autism can be associated with other disorders that affect the brain, such as: * Fragile X syndrome * Mental retardation * Tuberous sclerosis	topic_aut
73892	1	354804	5	NULL	NULL	0	NULL	autism	MedicalFinding		develops					seizures	MedicalFinding				NULL	few people	0	NULL	NULL	NULL	NULL	NULL	Some people with autism will develop seizures	topic_aut
74032	1	354806	7	NULL	NULL	0	NULL	bipolar disorder	MedicalFinding	people with	have					heart disease	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	People diagnosed with bipolar disorder are more likely to have certain other health problems, including heart disease, thyroid problems and obesity.	topic_bd
74033	2	354806	7	NULL	NULL	0	NULL	bipolar disorder	MedicalFinding	people with	have					thyroid problems	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	People diagnosed with bipolar disorder are more likely to have certain other health problems, including heart disease, thyroid problems and obesity.	topic_bd
74034	3	354806	7	NULL	NULL	0	NULL	bipolar disorder	MedicalFinding	people with	have					obesity	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	People diagnosed with bipolar disorder are more likely to have certain other health problems, including heart disease, thyroid problems and obesity.	topic_bd
74035	1	354807	7	NULL	NULL	0	NULL	Lithium	Chemical		effective at					stabilizing mood	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Lithium (Lithobid, others) is effective at stabilizing mood and preventing the extreme highs and lows of certain categories of bipolar disorder and has been used for many years. 	topic_bd
74036	2	354807	7	NULL	NULL	0	NULL	Lithium	Chemical		prevent					bipolar disorder	MedicalFinding	extreme high of			NULL		0	NULL	NULL	NULL	NULL	NULL	Lithium (Lithobid, others) is effective at stabilizing mood and preventing the extreme highs and lows of certain categories of bipolar disorder and has been used for many years. 	topic_bd
74037	3	354807	7	NULL	NULL	0	NULL	Lithium	Chemical		prevent					bipolar disorder	MedicalFinding	extreme lows of			NULL		0	NULL	NULL	NULL	NULL	NULL	Lithium (Lithobid, others) is effective at stabilizing mood and preventing the extreme highs and lows of certain categories of bipolar disorder and has been used for many years. 	topic_bd
74038	1	354808	7	NULL	NULL	0	NULL	 valproic acid 	Chemical		is a type of					mood stabilizing medications	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	•\tAnticonvulsants. These mood stabilizing medications include valproic acid (Depakene), divalproex (Depakote) and lamotrigine (Lamictal). 	topic_bd
74039	2	354808	7	NULL	NULL	0	NULL	divalproex	Chemical		is a type of					mood stabilizing medications	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	•\tAnticonvulsants. These mood stabilizing medications include valproic acid (Depakene), divalproex (Depakote) and lamotrigine (Lamictal). 	topic_bd
74040	3	354808	7	NULL	NULL	0	NULL	lamotrigine	Chemical		is a type of					mood stabilizing medications	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	•\tAnticonvulsants. These mood stabilizing medications include valproic acid (Depakene), divalproex (Depakote) and lamotrigine (Lamictal). 	topic_bd
74041	4	354808	7	NULL	NULL	0	NULL	valproic acid	Chemical		is					Depakene	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	•\tAnticonvulsants. These mood stabilizing medications include valproic acid (Depakene), divalproex (Depakote) and lamotrigine (Lamictal). 	topic_bd
74042	5	354808	7	NULL	NULL	0	NULL	divalproex 	Chemical		is					Depakote	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	•\tAnticonvulsants. These mood stabilizing medications include valproic acid (Depakene), divalproex (Depakote) and lamotrigine (Lamictal). 	topic_bd
74043	6	354808	7	NULL	NULL	0	NULL	lamotrigine	Chemical		is					Lamictal	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	•\tAnticonvulsants. These mood stabilizing medications include valproic acid (Depakene), divalproex (Depakote) and lamotrigine (Lamictal). 	topic_bd
74044	1	354810	7	NULL	NULL	0	NULL	antidepressants	Chemical		trigger					manic episodes	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In some people with bipolar disorder, antidepressants can trigger manic episodes, but may be OK if taken along with a mood stabilizer.	topic_bd
74045	2	354810	7	NULL	NULL	0	NULL	statement 1	Process		occur in					bipolar disorder	MedicalFinding	people with			NULL		0	NULL	NULL	NULL	NULL	NULL	In some people with bipolar disorder, antidepressants can trigger manic episodes, but may be OK if taken along with a mood stabilizer.	topic_bd
74046	3	354810	7	NULL	NULL	NULL	NULL	statement 1	Process		does not occur					mood stabilizer	Chemical	along with			NULL		NULL	NULL	NULL	NULL	NULL	NULL	In some people with bipolar disorder, antidepressants can trigger manic episodes, but may be OK if taken along with a mood stabilizer.	topic_bd
74047	1	354811	7	NULL	NULL	0	NULL	olanzapine	Chemical		is a type of					antipsychotic medication	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Certain antipsychotic medications, such as olanzapine (Zyprexa), risperidone (Risperdal) and quetiapine (Seroquel), may help people who don't gain benefits from anticonvulsants.	topic_bd
74048	2	354811	7	NULL	NULL	0	NULL	risperidone	Chemical		is a type of					antipsychotic medication	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Certain antipsychotic medications, such as olanzapine (Zyprexa), risperidone (Risperdal) and quetiapine (Seroquel), may help people who don't gain benefits from anticonvulsants.	topic_bd
74049	3	354811	7	NULL	NULL	0	NULL	quetiapine	Chemical		is a type of					antipsychotic medication	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Certain antipsychotic medications, such as olanzapine (Zyprexa), risperidone (Risperdal) and quetiapine (Seroquel), may help people who don't gain benefits from anticonvulsants.	topic_bd
74050	4	354811	7	NULL	NULL	0	NULL	olanzapine 	Chemical		is					Zyprexa	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Certain antipsychotic medications, such as olanzapine (Zyprexa), risperidone (Risperdal) and quetiapine (Seroquel), may help people who don't gain benefits from anticonvulsants.	topic_bd
74051	5	354811	7	NULL	NULL	0	NULL	 risperidone	Chemical		is					Risperdal	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Certain antipsychotic medications, such as olanzapine (Zyprexa), risperidone (Risperdal) and quetiapine (Seroquel), may help people who don't gain benefits from anticonvulsants.	topic_bd
74052	6	354811	7	NULL	NULL	0	NULL	quetiapine	Chemical		is					Seroquel	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Certain antipsychotic medications, such as olanzapine (Zyprexa), risperidone (Risperdal) and quetiapine (Seroquel), may help people who don't gain benefits from anticonvulsants.	topic_bd
74053	1	354812	7	NULL	NULL	0	NULL	anti-anxiety medications	Chemical		help with		may			anxiety	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	•\tBenzodiazepines. These anti-anxiety medications may help with anxiety and improve sleep. Examples include clonazepam (Klonopin), lorazepam (Ativan), diazepam (Valium), chlordiazepoxide (Librium) and alprazolam (Xanax).	topic_bd
74054	2	354812	7	NULL	NULL	NULL	NULL	anti-anxiety medications	Chemical		improve		may			sleep	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	•\tBenzodiazepines. These anti-anxiety medications may help with anxiety and improve sleep. Examples include clonazepam (Klonopin), lorazepam (Ativan), diazepam (Valium), chlordiazepoxide (Librium) and alprazolam (Xanax).	topic_bd
74055	3	354812	7	NULL	NULL	0	NULL	clonazepam	Chemical		is a type of					anti-anxiety medications	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	•\tBenzodiazepines. These anti-anxiety medications may help with anxiety and improve sleep. Examples include clonazepam (Klonopin), lorazepam (Ativan), diazepam (Valium), chlordiazepoxide (Librium) and alprazolam (Xanax).	topic_bd
74056	4	354812	7	NULL	NULL	0	NULL	lorazepam	Chemical		is a type of					anti-anxiety medications	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	•\tBenzodiazepines. These anti-anxiety medications may help with anxiety and improve sleep. Examples include clonazepam (Klonopin), lorazepam (Ativan), diazepam (Valium), chlordiazepoxide (Librium) and alprazolam (Xanax).	topic_bd
74057	5	354812	7	NULL	NULL	0	NULL	diazepam	Chemical		is a type of					anti-anxiety medications	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	•\tBenzodiazepines. These anti-anxiety medications may help with anxiety and improve sleep. Examples include clonazepam (Klonopin), lorazepam (Ativan), diazepam (Valium), chlordiazepoxide (Librium) and alprazolam (Xanax).	topic_bd
74058	6	354812	7	NULL	NULL	0	NULL	chlordiazepoxide	Chemical		is a type of					anti-anxiety medications	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	•\tBenzodiazepines. These anti-anxiety medications may help with anxiety and improve sleep. Examples include clonazepam (Klonopin), lorazepam (Ativan), diazepam (Valium), chlordiazepoxide (Librium) and alprazolam (Xanax).	topic_bd
74059	7	354812	7	NULL	NULL	0	NULL	alprazolam	Chemical		is a type of					anti-anxiety medications	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	•\tBenzodiazepines. These anti-anxiety medications may help with anxiety and improve sleep. Examples include clonazepam (Klonopin), lorazepam (Ativan), diazepam (Valium), chlordiazepoxide (Librium) and alprazolam (Xanax).	topic_bd
74060	8	354812	7	NULL	NULL	0	NULL	 clonazepam	Chemical		is					Klonopin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	•\tBenzodiazepines. These anti-anxiety medications may help with anxiety and improve sleep. Examples include clonazepam (Klonopin), lorazepam (Ativan), diazepam (Valium), chlordiazepoxide (Librium) and alprazolam (Xanax).	topic_bd
74061	9	354812	7	NULL	NULL	0	NULL	lorazepam	Chemical		is					Ativan	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	•\tBenzodiazepines. These anti-anxiety medications may help with anxiety and improve sleep. Examples include clonazepam (Klonopin), lorazepam (Ativan), diazepam (Valium), chlordiazepoxide (Librium) and alprazolam (Xanax).	topic_bd
74062	10	354812	7	NULL	NULL	0	NULL	diazepam	Chemical		is					Valium	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	•\tBenzodiazepines. These anti-anxiety medications may help with anxiety and improve sleep. Examples include clonazepam (Klonopin), lorazepam (Ativan), diazepam (Valium), chlordiazepoxide (Librium) and alprazolam (Xanax).	topic_bd
74063	11	354812	7	NULL	NULL	0	NULL	chlordiazepoxide	Chemical		is					Librium	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	•\tBenzodiazepines. These anti-anxiety medications may help with anxiety and improve sleep. Examples include clonazepam (Klonopin), lorazepam (Ativan), diazepam (Valium), chlordiazepoxide (Librium) and alprazolam (Xanax).	topic_bd
74064	12	354812	7	NULL	NULL	0	NULL	alprazolam	Chemical		is					Xanax	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	•\tBenzodiazepines. These anti-anxiety medications may help with anxiety and improve sleep. Examples include clonazepam (Klonopin), lorazepam (Ativan), diazepam (Valium), chlordiazepoxide (Librium) and alprazolam (Xanax).	topic_bd
74065	1	354814	7	NULL	NULL	0	NULL	Cyclothymia	MedicalFinding		is a mild form of					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Cyclothymia is a mild form of bipolar disorder. With cyclothymia, hypomania and depression can be disruptive, but the highs and lows are not as severe as they are with other types of bipolar disorder.	topic_bd
74066	2	354814	7	NULL	NULL	0	NULL	hypomania	MedicalFinding		can be					disruptive	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Cyclothymia is a mild form of bipolar disorder. With cyclothymia, hypomania and depression can be disruptive, but the highs and lows are not as severe as they are with other types of bipolar disorder.	topic_bd
74067	3	354814	7	NULL	NULL	0	NULL	depression	MedicalFinding		can be					disruptive	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Cyclothymia is a mild form of bipolar disorder. With cyclothymia, hypomania and depression can be disruptive, but the highs and lows are not as severe as they are with other types of bipolar disorder.	topic_bd
74068	4	354814	7	NULL	NULL	0	NULL	statement 2	Process		along with					cyclothymia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Cyclothymia is a mild form of bipolar disorder. With cyclothymia, hypomania and depression can be disruptive, but the highs and lows are not as severe as they are with other types of bipolar disorder.	topic_bd
74069	5	354814	7	NULL	NULL	0	NULL	statement 3	Process		along with					cyclothymia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Cyclothymia is a mild form of bipolar disorder. With cyclothymia, hypomania and depression can be disruptive, but the highs and lows are not as severe as they are with other types of bipolar disorder.	topic_bd
74070	6	354814	7	NULL	NULL	0	NULL	Cyclothymia	MedicalFinding	highs of	is not as severe as					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Cyclothymia is a mild form of bipolar disorder. With cyclothymia, hypomania and depression can be disruptive, but the highs and lows are not as severe as they are with other types of bipolar disorder.	topic_bd
74071	7	354814	7	NULL	NULL	0	NULL	Cyclothymia	MedicalFinding	lows of	is not as severe as					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Cyclothymia is a mild form of bipolar disorder. With cyclothymia, hypomania and depression can be disruptive, but the highs and lows are not as severe as they are with other types of bipolar disorder.	topic_bd
74086	1	354816	7	NULL	NULL	NULL	NULL	bipolar disorder	MedicalFinding	people with	have					brain	OrganismPart	physical changes in			NULL		NULL	NULL	NULL	NULL	NULL	NULL	People with bipolar disorder appear to have physical changes in their brains.	topic_bd
74087	1	354817	7	NULL	NULL	NULL	NULL	Imbalanced hormones	GP		involved in		may be			bipolar disorder	MedicalFinding	triggering			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Imbalanced hormones may be involved in causing or triggering bipolar disorder.	topic_bd
74088	2	354817	7	NULL	NULL	0	NULL	Imbalanced hormones	GP		involved in		may be			bipolar disorder	MedicalFinding	causing			NULL		0	NULL	NULL	NULL	NULL	NULL	Imbalanced hormones may be involved in causing or triggering bipolar disorder.	topic_bd
74089	1	354818	7	NULL	NULL	NULL	NULL	Stress	Process		play a role in		may			bipolar disorder	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Stress, abuse, significant loss or other traumatic experiences may play a role in bipolar disorder.	topic_bd
74090	2	354818	7	NULL	NULL	0	NULL	abuse	Process		play a role in		may			bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Stress, abuse, significant loss or other traumatic experiences may play a role in bipolar disorder.	topic_bd
74091	3	354818	7	NULL	NULL	NULL	NULL	traumatic experiences 	Process		play a role in		may			bipolar disorder	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Stress, abuse, significant loss or other traumatic experiences may play a role in bipolar disorder.	topic_bd
74092	1	354819	7	NULL	NULL	0	NULL	monoamines	Chemical		involved in		may be			BPD	MedicalFinding	pathophysiology of			NULL		0	NULL	NULL	NULL	NULL	NULL	Current data suggest that monoamines, acetylcholine, amino acids, cortisol, thyroid hormones, and melatonin may be involved in the pathophysiology of bipolar disorder (BPD).	topic_bd
74093	2	354819	7	NULL	NULL	0	NULL	acetylcholine	Chemical		involved in		may be			BPD	MedicalFinding	pathophysiology of			NULL		0	NULL	NULL	NULL	NULL	NULL	Current data suggest that monoamines, acetylcholine, amino acids, cortisol, thyroid hormones, and melatonin may be involved in the pathophysiology of bipolar disorder (BPD).	topic_bd
74094	3	354819	7	NULL	NULL	0	NULL	 amino acids	AminoAcid		involved in		may be			BPD	MedicalFinding	pathophysiology of			NULL		0	NULL	NULL	NULL	NULL	NULL	Current data suggest that monoamines, acetylcholine, amino acids, cortisol, thyroid hormones, and melatonin may be involved in the pathophysiology of bipolar disorder (BPD).	topic_bd
74095	4	354819	7	NULL	NULL	NULL	NULL	cortisol	Chemical		 involved in		may be			BPD	MedicalFinding	pathophysiology of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current data suggest that monoamines, acetylcholine, amino acids, cortisol, thyroid hormones, and melatonin may be involved in the pathophysiology of bipolar disorder (BPD).	topic_bd
74096	5	354819	7	NULL	NULL	NULL	NULL	thyroid hormones	Chemical		 involved in		may be			BPD	MedicalFinding	pathophysiology of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current data suggest that monoamines, acetylcholine, amino acids, cortisol, thyroid hormones, and melatonin may be involved in the pathophysiology of bipolar disorder (BPD).	topic_bd
74097	6	354819	7	NULL	NULL	0	NULL	melatonin	Chemical		involved in		may be			BPD	MedicalFinding	pathophysiology of			NULL		0	NULL	NULL	NULL	NULL	NULL	Current data suggest that monoamines, acetylcholine, amino acids, cortisol, thyroid hormones, and melatonin may be involved in the pathophysiology of bipolar disorder (BPD).	topic_bd
74098	7	354819	7	NULL	NULL	0	NULL	BPD	MedicalFinding		is					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Current data suggest that monoamines, acetylcholine, amino acids, cortisol, thyroid hormones, and melatonin may be involved in the pathophysiology of bipolar disorder (BPD).	topic_bd
74099	1	354820	7	NULL	NULL	0	NULL	acetylcholine	Chemical		is a type of					neurotransmitter	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The chemical compound acetylcholine (often abbreviated ACh) is a neurotransmitter	topic_bd
74100	2	354820	7	NULL	NULL	0	NULL	ACh	Chemical		is					acetylcholine	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The chemical compound acetylcholine (often abbreviated ACh) is a neurotransmitter	topic_bd
74101	3	354820	7	NULL	NULL	0	NULL	acetylcholine	Chemical		is a type of					chemical compound	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The chemical compound acetylcholine (often abbreviated ACh) is a neurotransmitter	topic_bd
74102	1	354821	7	NULL	NULL	0	NULL	Melatonin	GP		made by					pineal gland	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin is a hormone made by the pineal gland , a small gland in the brain. 	topic_bd
74103	2	354821	7	NULL	NULL	0	NULL	pineal gland	OrganismPart		is a type of					small gland	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin is a hormone made by the pineal gland , a small gland in the brain. 	topic_bd
74104	3	354821	7	NULL	NULL	0	NULL	Melatonin	GP		is a type of					hormone	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin is a hormone made by the pineal gland , a small gland in the brain. 	topic_bd
74105	1	354822	7	NULL	NULL	0	NULL	Antidepressants	Chemical		cause					TEM	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Antidepressants, stimulants, anticholinergics, steroids, and thyroid hormone have been reported to cause treatment-emergent mania (TEM) in BPD	topic_bd
74106	2	354822	7	NULL	NULL	0	NULL	stimulants	Chemical		cause					TEM	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Antidepressants, stimulants, anticholinergics, steroids, and thyroid hormone have been reported to cause treatment-emergent mania (TEM) in BPD	topic_bd
74107	3	354822	7	NULL	NULL	0	NULL	anticholinergics	Chemical		cause					TEM	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Antidepressants, stimulants, anticholinergics, steroids, and thyroid hormone have been reported to cause treatment-emergent mania (TEM) in BPD	topic_bd
74108	4	354822	7	NULL	NULL	0	NULL	steroids	Chemical		cause					TEM	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Antidepressants, stimulants, anticholinergics, steroids, and thyroid hormone have been reported to cause treatment-emergent mania (TEM) in BPD	topic_bd
74109	5	354822	7	NULL	NULL	0	NULL	 thyroid hormone	GP		cause					TEM	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Antidepressants, stimulants, anticholinergics, steroids, and thyroid hormone have been reported to cause treatment-emergent mania (TEM) in BPD	topic_bd
74110	6	354822	7	NULL	NULL	0	NULL	statement 1	Process		occur in					BPD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Antidepressants, stimulants, anticholinergics, steroids, and thyroid hormone have been reported to cause treatment-emergent mania (TEM) in BPD	topic_bd
74111	7	354822	7	NULL	NULL	0	NULL	statement 2	Process		occur in					BPD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Antidepressants, stimulants, anticholinergics, steroids, and thyroid hormone have been reported to cause treatment-emergent mania (TEM) in BPD	topic_bd
74112	8	354822	7	NULL	NULL	0	NULL	statement 3	Process		occur in					BPD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Antidepressants, stimulants, anticholinergics, steroids, and thyroid hormone have been reported to cause treatment-emergent mania (TEM) in BPD	topic_bd
74113	9	354822	7	NULL	NULL	0	NULL	statement 4	Process		occur in					BPD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Antidepressants, stimulants, anticholinergics, steroids, and thyroid hormone have been reported to cause treatment-emergent mania (TEM) in BPD	topic_bd
74114	10	354822	7	NULL	NULL	0	NULL	statement 5	Process		occur in					BPD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Antidepressants, stimulants, anticholinergics, steroids, and thyroid hormone have been reported to cause treatment-emergent mania (TEM) in BPD	topic_bd
74115	11	354822	7	NULL	NULL	0	NULL	TEM	MedicalFinding		is					 treatment-emergent mania	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Antidepressants, stimulants, anticholinergics, steroids, and thyroid hormone have been reported to cause treatment-emergent mania (TEM) in BPD	topic_bd
74116	1	354823	7	NULL	NULL	0	NULL	 anticholinergic agent 	Chemical		blocks					acetylcholine	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	An anticholinergic agent is a substance that blocks the neurotransmitter acetylcholine in the central and the peripheral nervous system.	topic_bd
74117	2	354823	7	NULL	NULL	0	NULL	statement 1	Process		occur in					central nervous system	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	An anticholinergic agent is a substance that blocks the neurotransmitter acetylcholine in the central and the peripheral nervous system.	topic_bd
74118	3	354823	7	NULL	NULL	0	NULL	statement 1	Process		occur in					peripheral nervous system	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	An anticholinergic agent is a substance that blocks the neurotransmitter acetylcholine in the central and the peripheral nervous system.	topic_bd
74119	4	354823	7	NULL	NULL	0	NULL	acetylcholine	Chemical		is a type of					neurotransmitter	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	An anticholinergic agent is a substance that blocks the neurotransmitter acetylcholine in the central and the peripheral nervous system.	topic_bd
74120	1	354825	7	NULL	NULL	NULL	NULL	HNF6	GP		function as					key regulators	GP				NULL		NULL	NULL	NULL	NULL	NULL	NULL	HNF6 and FOXA2 function as key regulators in human colorectal liver metastases.	topic_ccc
74121	2	354825	7	NULL	NULL	0	NULL	FOXA2	GP		function as					key regulators	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	HNF6 and FOXA2 function as key regulators in human colorectal liver metastases.	topic_ccc
74122	3	354825	7	NULL	NULL	0	NULL	statement 1	Process		occur in					 colorectal liver metastases	Process	human			NULL		0	NULL	NULL	NULL	NULL	NULL	HNF6 and FOXA2 function as key regulators in human colorectal liver metastases.	topic_ccc
74123	4	354825	7	NULL	NULL	NULL	NULL	statement 2	Process		occur in 					 colorectal liver metastases	Process	human			NULL		NULL	NULL	NULL	NULL	NULL	NULL	HNF6 and FOXA2 function as key regulators in human colorectal liver metastases.	topic_ccc
74124	1	354826	7	NULL	NULL	0	NULL	HNF6	GP		inhibit					cell cycle progression	Process				NULL	Caco-2 cell line	0	NULL	NULL	NULL	NULL	NULL	HNF6 inhibited cell cycle progression in the G2/M and G1 phase in Caco-2 and HepG2 cell lines	topic_ccc
74125	2	354826	7	NULL	NULL	0	NULL	HNF6	GP		inhibit					cell cycle progression	Process				NULL	HepG2 cell line	0	NULL	NULL	NULL	NULL	NULL	HNF6 inhibited cell cycle progression in the G2/M and G1 phase in Caco-2 and HepG2 cell lines	topic_ccc
74126	3	354826	7	NULL	NULL	0	NULL	statement 1	Process		occur in					G2/M phase	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	HNF6 inhibited cell cycle progression in the G2/M and G1 phase in Caco-2 and HepG2 cell lines	topic_ccc
74127	4	354826	7	NULL	NULL	0	NULL	statement 1	Process		occur in					G1 phase	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	HNF6 inhibited cell cycle progression in the G2/M and G1 phase in Caco-2 and HepG2 cell lines	topic_ccc
74128	5	354826	7	NULL	NULL	0	NULL	statement 2	Process		occur in					G2/M  phase	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	HNF6 inhibited cell cycle progression in the G2/M and G1 phase in Caco-2 and HepG2 cell lines	topic_ccc
74129	6	354826	7	NULL	NULL	0	NULL	statement 2	Process		occur in					G1 phase	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	HNF6 inhibited cell cycle progression in the G2/M and G1 phase in Caco-2 and HepG2 cell lines	topic_ccc
74130	1	354827	7	NULL	NULL	0	NULL	FOXA2	GP	functional knockdown of	recovered					HNF6 activity	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore functional knockdown of FOXA2 recovered HNF6 activity and inhibited growth of tumor-cells and may possibly represent a novel therapeutic target in primary and secondary liver malignancies.	topic_ccc
74131	2	354827	7	NULL	NULL	0	NULL	statement 1	Process		inhibit					tumor cells	Cell	growth of			NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore functional knockdown of FOXA2 recovered HNF6 activity and inhibited growth of tumor-cells and may possibly represent a novel therapeutic target in primary and secondary liver malignancies.	topic_ccc
74132	3	354827	7	NULL	NULL	0	NULL	FOXA2	GP		therapeutic target in		novel			primary liver malignancy	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore functional knockdown of FOXA2 recovered HNF6 activity and inhibited growth of tumor-cells and may possibly represent a novel therapeutic target in primary and secondary liver malignancies.	topic_ccc
74133	4	354827	7	NULL	NULL	0	NULL	FOXA2	GP		therapeutic target in 		novel			secondary liver malignancy	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore functional knockdown of FOXA2 recovered HNF6 activity and inhibited growth of tumor-cells and may possibly represent a novel therapeutic target in primary and secondary liver malignancies.	topic_ccc
74134	1	354828	7	NULL	NULL	NULL	NULL	FOXA2	GP	functional knockdown of	recovered					HNF6 activity	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Thus, functional knockdown of FOXA2 recovered HNF6 activity.	topic_ccc
74135	1	354830	7	NULL	NULL	0	NULL	Programmed cell death	Process		is called					apoptosis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Programmed cell death is also called apoptosis.	topic_ccc
74136	1	354831	7	NULL	NULL	0	NULL	TNF	Chemical	high dosage of	increase		significantly			apoptosis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	TNFα at a high dosage, a significant increase in the apoptosis rate was observed after 6 h and after 12 h in all dosage groups.	topic_ccc
74137	1	354832	7	NULL	NULL	0	NULL	CD95	Cell		induce					apoptosis	Process				NULL	liver metastases of colorectal carcinoma	0	NULL	NULL	NULL	NULL	NULL	CD95 and TNFα-induced apoptosis in liver metastases of colorectal carcinoma.As apoptosis contributes to the overall sensitivity to radiotherapy or chemotherapy, a better understanding of the apoptotic process in metastatic tumour tissues is necessary.	topic_ccc
74138	2	354832	7	NULL	NULL	0	NULL	TNF	Chemical		induce 					apoptosis	Process				NULL	liver metastases of colorectal carcinoma	0	NULL	NULL	NULL	NULL	NULL	CD95 and TNFα-induced apoptosis in liver metastases of colorectal carcinoma.As apoptosis contributes to the overall sensitivity to radiotherapy or chemotherapy, a better understanding of the apoptotic process in metastatic tumour tissues is necessary.	topic_ccc
74139	1	354836	7	NULL	NULL	0	NULL	 P-LVD	OrganismPart	high expression of	associated with					stage I colorectal cancer	MedicalFinding	shorter disease-free interval in			NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, high P-LVD and high VEGF expression were significant negative prognostic parameters associated with a shorter disease-free interval in stage I colorectal cancer	topic_ccc
74140	2	354836	7	NULL	NULL	NULL	NULL	VEGF	GP	high expression of	associated with					stage I colorectal cancer	MedicalFinding	shorter disease-free interval in			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Moreover, high P-LVD and high VEGF expression were significant negative prognostic parameters associated with a shorter disease-free interval in stage I colorectal cancer	topic_ccc
74141	3	354836	7	NULL	NULL	0	NULL	P-LVD	OrganismPart		is a type of					negative prognostic parameters	QuantityOrMeasure				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, high P-LVD and high VEGF expression were significant negative prognostic parameters associated with a shorter disease-free interval in stage I colorectal cancer	topic_ccc
74142	4	354836	7	NULL	NULL	0	NULL	VEGF	GP		is a type of					negative prognostic parameters	QuantityOrMeasure				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, high P-LVD and high VEGF expression were significant negative prognostic parameters associated with a shorter disease-free interval in stage I colorectal cancer	topic_ccc
74143	1	354837	7	NULL	NULL	0	NULL	P-LVD	OrganismPart		used as a tool 					stage I colorectal cancer	MedicalFinding	to identify			NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions If our findings are further confirmed in other studies, the assessment of P-LVD on surgical specimens might be used as a tool to identify patients with stage I colorectal cancer 	topic_ccc
74276	1	354838	7	NULL	NULL	0	NULL	VEGF	GP	high expression of	associate with					stage I colorectal cancer	MedicalFinding	shorter disease-free interval in			NULL		0	NULL	NULL	NULL	NULL	NULL	 high VEGF expression were significant negative prognostic parameters associated with a shorter disease-free interval in stage I colorectal cancer.	topic_ccc
74277	2	354838	7	NULL	NULL	NULL	NULL	VEGF	GP	high expression of	is a type of					negative prognostic parameters	QuantityOrMeasure				NULL		NULL	NULL	NULL	NULL	NULL	NULL	 high VEGF expression were significant negative prognostic parameters associated with a shorter disease-free interval in stage I colorectal cancer.	topic_ccc
73893	1	354839	5	NULL	NULL	0	NULL	delusions	MedicalFinding		is a symptom of					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Over two-thirds of patients with NMDAR antibody encephalitis, and some with potassium channel antibody-associated limbic encephalitis, have prominent psychiatric symptoms, or may present to psychiatric services in the first instance. The psychiatric symptoms are those seen in schizophrenia including delusions, hallucinations, and catatonic movement disorder.	topic_sch
73894	2	354839	5	NULL	NULL	0	NULL	hallucinations	MedicalFinding		is a symptom of					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Over two-thirds of patients with NMDAR antibody encephalitis, and some with potassium channel antibody-associated limbic encephalitis, have prominent psychiatric symptoms, or may present to psychiatric services in the first instance. The psychiatric symptoms are those seen in schizophrenia including delusions, hallucinations, and catatonic movement disorder.	topic_sch
73895	3	354839	5	NULL	NULL	0	NULL	catatonic movement disorder	MedicalFinding		is a symptom of					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Over two-thirds of patients with NMDAR antibody encephalitis, and some with potassium channel antibody-associated limbic encephalitis, have prominent psychiatric symptoms, or may present to psychiatric services in the first instance. The psychiatric symptoms are those seen in schizophrenia including delusions, hallucinations, and catatonic movement disorder.	topic_sch
73896	1	354840	5	NULL	NULL	0	NULL	NDUFV2	GP		is					NADH dehydrogenase ubiquinone flavoprotein 2	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	NADH dehydrogenase ubiquinone flavoprotein 2 (NDUFV2), encoding a subunit of mitochondrial complex I, is a candidate gene for several neuronal diseases; schizophrenia, bipolar disorder and Parkinson disease (PD). 	topic_sch
73897	2	354840	5	NULL	NULL	0	NULL	NDUFV2	GP		encodes					mitochondrial complex I	GP	subunit of			NULL		0	NULL	NULL	NULL	NULL	NULL	NADH dehydrogenase ubiquinone flavoprotein 2 (NDUFV2), encoding a subunit of mitochondrial complex I, is a candidate gene for several neuronal diseases; schizophrenia, bipolar disorder and Parkinson disease (PD). 	topic_sch
73898	3	354840	5	NULL	NULL	0	NULL	NDUFV2	GP		is a candidate gene for					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	NADH dehydrogenase ubiquinone flavoprotein 2 (NDUFV2), encoding a subunit of mitochondrial complex I, is a candidate gene for several neuronal diseases; schizophrenia, bipolar disorder and Parkinson disease (PD). 	topic_sch
73899	4	354840	5	NULL	NULL	0	NULL	NDUFV2	GP		is a candidate gene for					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	NADH dehydrogenase ubiquinone flavoprotein 2 (NDUFV2), encoding a subunit of mitochondrial complex I, is a candidate gene for several neuronal diseases; schizophrenia, bipolar disorder and Parkinson disease (PD). 	topic_sch
73900	5	354840	5	NULL	NULL	0	NULL	NDUFV2	GP		is a candidate gene for					Parkinson disease	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	NADH dehydrogenase ubiquinone flavoprotein 2 (NDUFV2), encoding a subunit of mitochondrial complex I, is a candidate gene for several neuronal diseases; schizophrenia, bipolar disorder and Parkinson disease (PD). 	topic_sch
73901	6	354840	5	NULL	NULL	0	NULL	PD	MedicalFinding		is					Parkinson disease	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	NADH dehydrogenase ubiquinone flavoprotein 2 (NDUFV2), encoding a subunit of mitochondrial complex I, is a candidate gene for several neuronal diseases; schizophrenia, bipolar disorder and Parkinson disease (PD). 	topic_sch
73902	7	354840	5	NULL	NULL	0	NULL	schizophrenia	MedicalFinding		is a type of					neuronal disease	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	NADH dehydrogenase ubiquinone flavoprotein 2 (NDUFV2), encoding a subunit of mitochondrial complex I, is a candidate gene for several neuronal diseases; schizophrenia, bipolar disorder and Parkinson disease (PD). 	topic_sch
73903	8	354840	5	NULL	NULL	0	NULL	bipolar disorder	MedicalFinding		is a type of					neuronal disease	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	NADH dehydrogenase ubiquinone flavoprotein 2 (NDUFV2), encoding a subunit of mitochondrial complex I, is a candidate gene for several neuronal diseases; schizophrenia, bipolar disorder and Parkinson disease (PD). 	topic_sch
73904	9	354840	5	NULL	NULL	0	NULL	Parkinson disease	MedicalFinding		is a type of					neuronal disease	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	NADH dehydrogenase ubiquinone flavoprotein 2 (NDUFV2), encoding a subunit of mitochondrial complex I, is a candidate gene for several neuronal diseases; schizophrenia, bipolar disorder and Parkinson disease (PD). 	topic_sch
73905	1	354842	5	NULL	NULL	0	NULL	improper inhibitory control	MedicalFinding		is involved in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	To explore this issue, we examined visual and visuomotor processing in schizophrenia, utilizing an illusion known as the Roelofs effect. These results provide evidence for a hypothesis of improper inhibitory control as a common mechanism underpinning abnormal visual and visuomotor processes in this mental disorder.	topic_sch
73906	1	354844	5	NULL	NULL	0	NULL	physical capacity	Process		is lower in					schizophrenic patients	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	The (schizophrenic) patients exhibited significantly higher RQ on submaximal workloads and lower physical capacity. A significant lower calculated VO(2-max) remained after correction for body weight and fat free mass (FFM). Energy expenditure did not differ on fixed workloads.	topic_sch
73907	2	354844	5	NULL	NULL	0	NULL	RQ	QuantityOrMeasure		is higher in		significantly			schizophrenic patients	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	The (schizophrenic) patients exhibited significantly higher RQ on submaximal workloads and lower physical capacity. A significant lower calculated VO(2-max) remained after correction for body weight and fat free mass (FFM). Energy expenditure did not differ on fixed workloads.	topic_sch
73908	1	354845	5	NULL	NULL	0	NULL	hippocampal atrophy	MedicalFinding		is a type of					morphological manifestation	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	NULL	NULL	One morphological manifestation of schizophrenia is hippocampal atrophy.	topic_sch
73909	2	354845	5	NULL	NULL	0	NULL	hippocampal atrophy	MedicalFinding		occurs in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	One morphological manifestation of schizophrenia is hippocampal atrophy.	topic_sch
74191	1	354846	11	NULL	NULL	0	NULL	Staphylococcus aureus	Organism	Methicillin-resistant	is responsible for					 infections	Process	 humans			NULL		0	NULL	NULL	NULL	NULL	NULL	Methicillin-resistant Staphylococcus aureus (MRSA) is a bacterium responsible for several difficult-to-treat infections in humans	topic_mrs
74192	2	354846	11	NULL	NULL	0	NULL	Staphylococcus aureus	Organism	Methicillin-resistant	is a					bacterium	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Methicillin-resistant Staphylococcus aureus (MRSA) is a bacterium responsible for several difficult-to-treat infections in humans	topic_mrs
73911	1	354847	5	NULL	NULL	NULL	NULL	Glx	Chemical	lower levels of	corelates with					impaired cognition	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although not reduced in schizophrenia as a group, lower Glx levels correlates with impaired cognition in the illness. 	topic_sch
74193	1	354847	5	11	NULL	NULL	NULL	Glx	Chemical	lower levels of	correlates with					impaired cognition	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although not reduced in schizophrenia as a group, lower Glx levels correlates with impaired cognition in the illness. 	topic_sch
74197	1	354847	5	11	NULL	0	NULL	 Glx	Chemical	lower levels of	occurs in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Although not reduced in schizophrenia as a group, lower Glx levels correlates with impaired cognition in the illness. 	topic_sch
73912	1	354849	5	NULL	NULL	0	NULL	D-serine	AminoAcid		is a coagonist of					NMDA receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The NMDA receptor coagonist D-serine is important in a number of different processes in the central nervous system, ranging from synaptic plasticity to disease states, including schizophrenia. 	topic_sch
73913	2	354849	5	11	NULL	NULL	NULL	D-serine	AminoAcid		plays a role in		different processes of			central nervous system	OrganismPart				NULL		NULL	NULL	NULL	NULL	NULL	NULL	The NMDA receptor coagonist D-serine is important in a number of different processes in the central nervous system, ranging from synaptic plasticity to disease states, including schizophrenia. 	topic_sch
73914	3	354849	5	NULL	NULL	0	NULL	D-serine	AminoAcid		plays a role in		important			synaptic plasticity	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The NMDA receptor coagonist D-serine is important in a number of different processes in the central nervous system, ranging from synaptic plasticity to disease states, including schizophrenia. 	topic_sch
73915	4	354849	5	NULL	NULL	0	NULL	D-serine	AminoAcid		plays a role in		important			schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The NMDA receptor coagonist D-serine is important in a number of different processes in the central nervous system, ranging from synaptic plasticity to disease states, including schizophrenia. 	topic_sch
74205	1	354849	5	11	NULL	0	NULL	 D-serine	AminoAcid		is a coagonist of 					NMDA receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The NMDA receptor coagonist D-serine is important in a number of different processes in the central nervous system, ranging from synaptic plasticity to disease states, including schizophrenia. 	topic_sch
74214	1	354849	5	11	NULL	NULL	NULL	D-serine	AminoAcid		plays a role in		important			central nervous system	OrganismPart	different processes in			NULL		NULL	NULL	NULL	NULL	NULL	NULL	The NMDA receptor coagonist D-serine is important in a number of different processes in the central nervous system, ranging from synaptic plasticity to disease states, including schizophrenia. 	topic_sch
74223	1	354849	5	11	NULL	0	NULL	D-serine	AminoAcid		plays a role in					synaptic plasticity	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The NMDA receptor coagonist D-serine is important in a number of different processes in the central nervous system, ranging from synaptic plasticity to disease states, including schizophrenia. 	topic_sch
74224	1	354849	5	11	NULL	0	NULL	D-serine	AminoAcid		plays a role in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The NMDA receptor coagonist D-serine is important in a number of different processes in the central nervous system, ranging from synaptic plasticity to disease states, including schizophrenia. 	topic_sch
76328	1	354850	11	NULL	NULL	0	NULL	Meticillin	Chemical		is also known as					methicillin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Meticillin  or methicillin  is a narrow-spectrum beta-lactam antibiotic of the penicillin class. 	topic_mrs
76329	2	354850	11	NULL	NULL	0	NULL	Meticillin	Chemical		is a type of 					 narrow-spectrum beta-lactam antibiotic 	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Meticillin  or methicillin  is a narrow-spectrum beta-lactam antibiotic of the penicillin class. 	topic_mrs
76330	3	354850	11	NULL	NULL	0	NULL	Meticillin	Chemical		is a class of					penicillin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Meticillin  or methicillin  is a narrow-spectrum beta-lactam antibiotic of the penicillin class. 	topic_mrs
74225	1	354851	11	NULL	NULL	0	NULL	Nafcillin sodium	Chemical		is a type of 					beta-lactam antibiotic	Chemical	narrow-spectrum			NULL		0	NULL	NULL	NULL	NULL	NULL	Nafcillin sodium is a narrow-spectrum beta-lactam antibiotic of the penicillin class. As a beta-lactamase-resistant penicillin, it is used to treat infections caused by Gram-positive bacteria, in particular, species of staphylococci that are resistant to other penicillins.	topic_mrs
74226	2	354851	11	NULL	NULL	0	NULL	Nafcillin sodium	Chemical		is a type of 					penicillin	Chemical	beta-lactamase-resistant 			NULL		0	NULL	NULL	NULL	NULL	NULL	Nafcillin sodium is a narrow-spectrum beta-lactam antibiotic of the penicillin class. As a beta-lactamase-resistant penicillin, it is used to treat infections caused by Gram-positive bacteria, in particular, species of staphylococci that are resistant to other penicillins.	topic_mrs
74227	3	354851	11	NULL	NULL	0	NULL	Nafcillin sodium	Chemical		 is used to treat					infections	Process	caused by staphylococci			NULL		0	NULL	NULL	NULL	NULL	NULL	Nafcillin sodium is a narrow-spectrum beta-lactam antibiotic of the penicillin class. As a beta-lactamase-resistant penicillin, it is used to treat infections caused by Gram-positive bacteria, in particular, species of staphylococci that are resistant to other penicillins.	topic_mrs
76331	1	354852	11	NULL	NULL	0	NULL	Clindamycin	Chemical		is a type of 					lincosamide antibiotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Clindamycin  is a lincosamide antibiotic.	topic_mrs
76332	1	354853	11	NULL	NULL	0	NULL	Dicloxacillin	Chemical		is a type of 					 narrow spectrum beta-lactam antibiotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Dicloxacillin  is a narrow spectrum beta-lactam antibiotic of the penicillin class	topic_mrs
76333	2	354853	11	NULL	NULL	0	NULL	Dicloxacillin	Chemical		is a class of					penicillin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Dicloxacillin  is a narrow spectrum beta-lactam antibiotic of the penicillin class	topic_mrs
76334	1	354854	11	NULL	NULL	0	NULL	β-Lactam antibiotics	Chemical		contains					β-lactam nucleus	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	β-Lactam antibiotics are a broad class of antibiotics, consisting of all antibiotic agents that contains a β-lactam nucleus in its molecular structure	topic_mrs
76335	1	354855	11	NULL	NULL	0	NULL	Penicillin	Chemical		is a group of					antibiotics	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Penicillin is a group of antibiotics derived from Penicillium fungi.	topic_mrs
76336	2	354855	11	NULL	NULL	0	NULL	Penicillin	Chemical		is derived from					Penicillium fungi	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Penicillin is a group of antibiotics derived from Penicillium fungi.	topic_mrs
73916	1	354856	5	NULL	NULL	0	NULL	Amphetamine	Chemical		improve					cognition	Process				NULL	schizophrenia patients	0	NULL	NULL	NULL	NULL	NULL	Amphetamine can improve cognition in healthy subjects and patients with schizophrenia, attention-deficit hyperactivity disorder (ADHD), and other neuropsychiatric diseases; higher doses, however, can impair cognitive function, especially those mediated by the prefrontal cortex (PFC). 	topic_sch
73917	2	354856	5	NULL	NULL	0	NULL	Amphetamine	Chemical		improve					cognition	Process				NULL	healthy subjects	0	NULL	NULL	NULL	NULL	NULL	Amphetamine can improve cognition in healthy subjects and patients with schizophrenia, attention-deficit hyperactivity disorder (ADHD), and other neuropsychiatric diseases; higher doses, however, can impair cognitive function, especially those mediated by the prefrontal cortex (PFC). 	topic_sch
73918	3	354856	5	NULL	NULL	0	NULL	Amphetamine	Chemical		improve					cognition	Process				NULL	ADHD patients	0	NULL	NULL	NULL	NULL	NULL	Amphetamine can improve cognition in healthy subjects and patients with schizophrenia, attention-deficit hyperactivity disorder (ADHD), and other neuropsychiatric diseases; higher doses, however, can impair cognitive function, especially those mediated by the prefrontal cortex (PFC). 	topic_sch
73919	4	354856	5	NULL	NULL	0	NULL	ADHD	MedicalFinding		is					attention-deficit hyperactivity disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Amphetamine can improve cognition in healthy subjects and patients with schizophrenia, attention-deficit hyperactivity disorder (ADHD), and other neuropsychiatric diseases; higher doses, however, can impair cognitive function, especially those mediated by the prefrontal cortex (PFC). 	topic_sch
73920	5	354856	5	NULL	NULL	0	NULL	Amphetamine	Chemical	higher doses of	impair					cognitive function	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Amphetamine can improve cognition in healthy subjects and patients with schizophrenia, attention-deficit hyperactivity disorder (ADHD), and other neuropsychiatric diseases; higher doses, however, can impair cognitive function, especially those mediated by the prefrontal cortex (PFC). 	topic_sch
73921	6	354856	5	NULL	NULL	0	NULL	cognitive function	Process		is mediated by					prefrontal cortex	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Amphetamine can improve cognition in healthy subjects and patients with schizophrenia, attention-deficit hyperactivity disorder (ADHD), and other neuropsychiatric diseases; higher doses, however, can impair cognitive function, especially those mediated by the prefrontal cortex (PFC). 	topic_sch
73922	7	354856	5	NULL	NULL	0	NULL	Amphetamine	Chemical	higher doses of	impair					statement 6	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Amphetamine can improve cognition in healthy subjects and patients with schizophrenia, attention-deficit hyperactivity disorder (ADHD), and other neuropsychiatric diseases; higher doses, however, can impair cognitive function, especially those mediated by the prefrontal cortex (PFC). 	topic_sch
73923	8	354856	5	NULL	NULL	0	NULL	PFC	OrganismPart		is					prefrontal cortex	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Amphetamine can improve cognition in healthy subjects and patients with schizophrenia, attention-deficit hyperactivity disorder (ADHD), and other neuropsychiatric diseases; higher doses, however, can impair cognitive function, especially those mediated by the prefrontal cortex (PFC). 	topic_sch
73924	1	354858	5	NULL	NULL	0	NULL	Glutamate	Chemical		is present in					prefrontal cortex	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamate in the prefrontal cortex (PFC) plays a significant role in several mental illnesses, including schizophrenia, addiction and anxiety. 	topic_sch
73925	2	354858	5	NULL	NULL	0	NULL	PFC	OrganismPart		is					prefrontal cortex	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamate in the prefrontal cortex (PFC) plays a significant role in several mental illnesses, including schizophrenia, addiction and anxiety. 	topic_sch
73926	3	354858	5	NULL	NULL	0	NULL	Glutamate	Chemical		plays a role in		important			schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamate in the prefrontal cortex (PFC) plays a significant role in several mental illnesses, including schizophrenia, addiction and anxiety. 	topic_sch
73927	4	354858	5	NULL	NULL	0	NULL	Glutamate	Chemical		plays a role in		important			addiction	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamate in the prefrontal cortex (PFC) plays a significant role in several mental illnesses, including schizophrenia, addiction and anxiety. 	topic_sch
73928	5	354858	5	NULL	NULL	0	NULL	Glutamate	Chemical		plays a role in		important			anxiety	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamate in the prefrontal cortex (PFC) plays a significant role in several mental illnesses, including schizophrenia, addiction and anxiety. 	topic_sch
76337	1	354859	11	NULL	NULL	0	NULL	β-Lactam antibiotics	Chemical		contains					 β-lactam nucleus	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	β-Lactam antibiotics are a broad class of antibiotics, consisting of all antibiotic agents that contains a β-lactam nucleus in its molecular structure. This includes penicillin derivatives (penams)  cephalosporins (cephems)	topic_mrs
76338	2	354859	11	NULL	NULL	0	NULL	β-Lactam antibiotics	Chemical		includes					cephalosporins 	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	β-Lactam antibiotics are a broad class of antibiotics, consisting of all antibiotic agents that contains a β-lactam nucleus in its molecular structure. This includes penicillin derivatives (penams)  cephalosporins (cephems)	topic_mrs
76339	3	354859	11	NULL	NULL	0	NULL	penams	Chemical		is a derivative of					penicillin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	β-Lactam antibiotics are a broad class of antibiotics, consisting of all antibiotic agents that contains a β-lactam nucleus in its molecular structure. This includes penicillin derivatives (penams)  cephalosporins (cephems)	topic_mrs
76340	4	354859	11	NULL	NULL	0	NULL	cephalosporins 	Chemical		is also known as					cephems	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	β-Lactam antibiotics are a broad class of antibiotics, consisting of all antibiotic agents that contains a β-lactam nucleus in its molecular structure. This includes penicillin derivatives (penams)  cephalosporins (cephems)	topic_mrs
73929	1	354860	5	NULL	NULL	0	NULL	STOP	GP		is a type of					microtubule-associated protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The deletion of microtubule-associated protein STOP leads to neuroanatomical, biochemical and severe behavioral alterations in mice, partly alleviated by antipsychotics. Therefore, STOP knockout (KO) mice have been proposed as a model of some schizophrenia-like symptoms. 	topic_sch
73930	2	354860	5	NULL	NULL	0	NULL	STOP	GP	deletion of	leads to					neuroanatomical alterations	MedicalFinding				NULL	mice	0	NULL	NULL	NULL	NULL	NULL	The deletion of microtubule-associated protein STOP leads to neuroanatomical, biochemical and severe behavioral alterations in mice, partly alleviated by antipsychotics. Therefore, STOP knockout (KO) mice have been proposed as a model of some schizophrenia-like symptoms. 	topic_sch
73931	3	354860	5	NULL	NULL	0	NULL	STOP	GP	deletion of	leads to					biochemical alterations	MedicalFinding				NULL	mice	0	NULL	NULL	NULL	NULL	NULL	The deletion of microtubule-associated protein STOP leads to neuroanatomical, biochemical and severe behavioral alterations in mice, partly alleviated by antipsychotics. Therefore, STOP knockout (KO) mice have been proposed as a model of some schizophrenia-like symptoms. 	topic_sch
73932	4	354860	5	NULL	NULL	0	NULL	STOP	GP	deletion of	leads to					bihavioral alterations	MedicalFinding	severe			NULL	mice	0	NULL	NULL	NULL	NULL	NULL	The deletion of microtubule-associated protein STOP leads to neuroanatomical, biochemical and severe behavioral alterations in mice, partly alleviated by antipsychotics. Therefore, STOP knockout (KO) mice have been proposed as a model of some schizophrenia-like symptoms. 	topic_sch
73934	5	354860	5	NULL	NULL	0	NULL	statement 2	Process		is alleviated by		partly			antipsychotics	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The deletion of microtubule-associated protein STOP leads to neuroanatomical, biochemical and severe behavioral alterations in mice, partly alleviated by antipsychotics. Therefore, STOP knockout (KO) mice have been proposed as a model of some schizophrenia-like symptoms. 	topic_sch
73935	6	354860	5	NULL	NULL	0	NULL	statement 3	Process		is alleviated by		partly			antipsychotics	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The deletion of microtubule-associated protein STOP leads to neuroanatomical, biochemical and severe behavioral alterations in mice, partly alleviated by antipsychotics. Therefore, STOP knockout (KO) mice have been proposed as a model of some schizophrenia-like symptoms. 	topic_sch
73936	7	354860	5	NULL	NULL	0	NULL	statement 4	Process		is alleviated by		partly			antipsychotics	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The deletion of microtubule-associated protein STOP leads to neuroanatomical, biochemical and severe behavioral alterations in mice, partly alleviated by antipsychotics. Therefore, STOP knockout (KO) mice have been proposed as a model of some schizophrenia-like symptoms. 	topic_sch
74931	1	354861	11	NULL	NULL	NULL	NULL	Vancomycin	Chemical		is a type of 					glycopeptide antibiotic	Chemical				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Vancomycin is a glycopeptide antibiotic used in the prophylaxis and treatment of infections caused by Gram-positive bacteria	topic_mrs
74932	2	354861	11	NULL	NULL	NULL	NULL	Vancomycin	Chemical		is used in					prophylaxis	MedicalProcedure				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Vancomycin is a glycopeptide antibiotic used in the prophylaxis and treatment of infections caused by Gram-positive bacteria	topic_mrs
74933	3	354861	11	NULL	NULL	NULL	NULL	infections	MedicalFinding		is caused by					Gram-positive bacteria	Organism				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Vancomycin is a glycopeptide antibiotic used in the prophylaxis and treatment of infections caused by Gram-positive bacteria	topic_mrs
74934	4	354861	11	NULL	NULL	0	NULL	Vancomycin	Chemical		treats					 infections	Medical Finding				NULL		0	NULL	NULL	NULL	NULL	NULL	Vancomycin is a glycopeptide antibiotic used in the prophylaxis and treatment of infections caused by Gram-positive bacteria	topic_mrs
74935	1	354862	11	NULL	NULL	NULL	NULL	Glycopeptide  antibiotics	Chemical		is composed of					glycosylated cyclic nonribosomal peptides	Chemical				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glycopeptide antibiotics are a class of antibiotic drugs. The class is composed of glycosylated cyclic or polycyclic nonribosomal peptides. Significant glycopeptide antibiotics include vancomycin, teicoplanin, telavancin, bleomycin, ramoplanin, and decaplanin.	topic_mrs
74936	2	354862	11	NULL	NULL	0	NULL	Glycopeptide antibiotics	Chemical		is composed of					glycosylated polycyclic nonribosomal peptides	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Glycopeptide antibiotics are a class of antibiotic drugs. The class is composed of glycosylated cyclic or polycyclic nonribosomal peptides. Significant glycopeptide antibiotics include vancomycin, teicoplanin, telavancin, bleomycin, ramoplanin, and decaplanin.	topic_mrs
74937	3	354862	11	NULL	NULL	NULL	NULL	statement 1	Process		is an alternative to 					statement 2	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glycopeptide antibiotics are a class of antibiotic drugs. The class is composed of glycosylated cyclic or polycyclic nonribosomal peptides. Significant glycopeptide antibiotics include vancomycin, teicoplanin, telavancin, bleomycin, ramoplanin, and decaplanin.	topic_mrs
75202	4	354862	11	NULL	NULL	0	NULL	Glycopeptide antibiotics	Chemical		is a class of					antibiotic drugs	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Glycopeptide antibiotics are a class of antibiotic drugs. The class is composed of glycosylated cyclic or polycyclic nonribosomal peptides. Significant glycopeptide antibiotics include vancomycin, teicoplanin, telavancin, bleomycin, ramoplanin, and decaplanin.	topic_mrs
75203	5	354862	11	NULL	NULL	0	NULL	vancomycin	Chemical		is a type of					glycopeptide antibiotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Glycopeptide antibiotics are a class of antibiotic drugs. The class is composed of glycosylated cyclic or polycyclic nonribosomal peptides. Significant glycopeptide antibiotics include vancomycin, teicoplanin, telavancin, bleomycin, ramoplanin, and decaplanin.	topic_mrs
75204	6	354862	11	NULL	NULL	0	NULL	teicoplanin	Chemical		is a type of 					glycopeptide antibiotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Glycopeptide antibiotics are a class of antibiotic drugs. The class is composed of glycosylated cyclic or polycyclic nonribosomal peptides. Significant glycopeptide antibiotics include vancomycin, teicoplanin, telavancin, bleomycin, ramoplanin, and decaplanin.	topic_mrs
75205	7	354862	11	NULL	NULL	0	NULL	telavancin	Chemical		is a type of 					glycopeptide antibiotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Glycopeptide antibiotics are a class of antibiotic drugs. The class is composed of glycosylated cyclic or polycyclic nonribosomal peptides. Significant glycopeptide antibiotics include vancomycin, teicoplanin, telavancin, bleomycin, ramoplanin, and decaplanin.	topic_mrs
75206	8	354862	11	NULL	NULL	0	NULL	bleomycin	Chemical		is a type of 					glycopeptide antibiotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Glycopeptide antibiotics are a class of antibiotic drugs. The class is composed of glycosylated cyclic or polycyclic nonribosomal peptides. Significant glycopeptide antibiotics include vancomycin, teicoplanin, telavancin, bleomycin, ramoplanin, and decaplanin.	topic_mrs
75207	9	354862	11	NULL	NULL	0	NULL	ramoplanin	Chemical		is a type of 					glycopeptide antibiotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Glycopeptide antibiotics are a class of antibiotic drugs. The class is composed of glycosylated cyclic or polycyclic nonribosomal peptides. Significant glycopeptide antibiotics include vancomycin, teicoplanin, telavancin, bleomycin, ramoplanin, and decaplanin.	topic_mrs
75208	10	354862	11	NULL	NULL	0	NULL	decaplanin	Chemical		is a type of 					glycopeptide antibiotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Glycopeptide antibiotics are a class of antibiotic drugs. The class is composed of glycosylated cyclic or polycyclic nonribosomal peptides. Significant glycopeptide antibiotics include vancomycin, teicoplanin, telavancin, bleomycin, ramoplanin, and decaplanin.	topic_mrs
75209	1	354863	11	NULL	NULL	0	NULL	Teicoplanin	Chemical		is a type of 					antibiotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Teicoplanin is an antibiotic used in the prophylaxis and treatment of serious infections caused by Gram-positive bacteria, including methicillin-resistant Staphylococcus aureus	topic_mrs
75211	2	354863	11	NULL	NULL	0	NULL	Teicoplanin	Chemical		used in					prophylaxis	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Teicoplanin is an antibiotic used in the prophylaxis and treatment of serious infections caused by Gram-positive bacteria, including methicillin-resistant Staphylococcus aureus	topic_mrs
75217	3	354863	11	NULL	NULL	0	NULL	infections	MedicalFinding		caused by					Gram-positive bacteria	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Teicoplanin is an antibiotic used in the prophylaxis and treatment of serious infections caused by Gram-positive bacteria, including methicillin-resistant Staphylococcus aureus	topic_mrs
75218	4	354863	11	NULL	NULL	0	NULL	Teicoplanin	Chemical		treats					infections	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Teicoplanin is an antibiotic used in the prophylaxis and treatment of serious infections caused by Gram-positive bacteria, including methicillin-resistant Staphylococcus aureus	topic_mrs
74984	1	354864	11	NULL	NULL	0	NULL	fibrinogen	GP		is converted to 					fibrin	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulase is a protein produced by several microorganisms, which enables the conversion of fibrinogen to fibrin	topic_mrs
74985	2	354864	11	NULL	NULL	0	NULL	Coagulase	GP		enables					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulase is a protein produced by several microorganisms, which enables the conversion of fibrinogen to fibrin	topic_mrs
74986	3	354864	11	NULL	NULL	0	NULL	Coagulase	GP		produced by					microorganisms	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulase is a protein produced by several microorganisms, which enables the conversion of fibrinogen to fibrin	topic_mrs
75210	4	354864	11	NULL	NULL	0	NULL	Coagulase	GP		is a type of 					protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulase is a protein produced by several microorganisms, which enables the conversion of fibrinogen to fibrin	topic_mrs
74987	1	354865	11	NULL	NULL	NULL	NULL	Coagulase	GP		complex with					prothrombin	GP	in the blood			NULL		NULL	NULL	NULL	NULL	NULL	NULL	If negative, the plasma remains liquid....If positive (i.e., the suspect colony is S. aureus), the serum will coagulate...Coagulase reacts with prothrombin in the blood. The resulting complex is called staphylothrombin, which enables the enzyme protease to convert fibrinogen to fibrin. This results in clotting of the blood. 	topic_mrs
74988	2	354865	11	NULL	NULL	0	NULL	statement 1	Process		produces					staphylothrombin	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	If negative, the plasma remains liquid....If positive (i.e., the suspect colony is S. aureus), the serum will coagulate...Coagulase reacts with prothrombin in the blood. The resulting complex is called staphylothrombin, which enables the enzyme protease to convert fibrinogen to fibrin. This results in clotting of the blood. 	topic_mrs
74989	3	354865	11	NULL	NULL	0	NULL	fibrinogen	GP		convert to					fibrin	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	If negative, the plasma remains liquid....If positive (i.e., the suspect colony is S. aureus), the serum will coagulate...Coagulase reacts with prothrombin in the blood. The resulting complex is called staphylothrombin, which enables the enzyme protease to convert fibrinogen to fibrin. This results in clotting of the blood. 	topic_mrs
74990	4	354865	11	NULL	NULL	0	NULL	protease	GP		enables					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	If negative, the plasma remains liquid....If positive (i.e., the suspect colony is S. aureus), the serum will coagulate...Coagulase reacts with prothrombin in the blood. The resulting complex is called staphylothrombin, which enables the enzyme protease to convert fibrinogen to fibrin. This results in clotting of the blood. 	topic_mrs
74991	5	354865	11	NULL	NULL	0	NULL	staphylothrombin	GP		enables					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	If negative, the plasma remains liquid....If positive (i.e., the suspect colony is S. aureus), the serum will coagulate...Coagulase reacts with prothrombin in the blood. The resulting complex is called staphylothrombin, which enables the enzyme protease to convert fibrinogen to fibrin. This results in clotting of the blood. 	topic_mrs
74992	6	354865	11	NULL	NULL	0	NULL	statement 3	Process		resulted in					blood clotting	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	If negative, the plasma remains liquid....If positive (i.e., the suspect colony is S. aureus), the serum will coagulate...Coagulase reacts with prothrombin in the blood. The resulting complex is called staphylothrombin, which enables the enzyme protease to convert fibrinogen to fibrin. This results in clotting of the blood. 	topic_mrs
75212	7	354865	11	NULL	NULL	0	NULL	protease	GP		is a type of 					enzyme	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	If negative, the plasma remains liquid....If positive (i.e., the suspect colony is S. aureus), the serum will coagulate...Coagulase reacts with prothrombin in the blood. The resulting complex is called staphylothrombin, which enables the enzyme protease to convert fibrinogen to fibrin. This results in clotting of the blood. 	topic_mrs
74993	1	354868	11	NULL	NULL	NULL	NULL	Peptidoglycan	Chemical		is also known as					murein	Chemical				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Peptidoglycan, also known as murein, is a polymer consisting of sugars and amino acids 	topic_mrs
74994	2	354868	11	NULL	NULL	0	NULL	Peptidoglycan	Chemical		is a type of 					polymer	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Peptidoglycan, also known as murein, is a polymer consisting of sugars and amino acids 	topic_mrs
74995	3	354868	11	NULL	NULL	0	NULL	Peptidoglycan	Chemical		consisting of					sugars	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Peptidoglycan, also known as murein, is a polymer consisting of sugars and amino acids 	topic_mrs
74996	4	354868	11	NULL	NULL	0	NULL	Peptidoglycan	Chemical		consisting of					amino acids	amino acid				NULL		0	NULL	NULL	NULL	NULL	NULL	Peptidoglycan, also known as murein, is a polymer consisting of sugars and amino acids 	topic_mrs
75000	5	354868	11	NULL	NULL	NULL	NULL	statement 3	Process		occurs along with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Peptidoglycan, also known as murein, is a polymer consisting of sugars and amino acids 	topic_mrs
75001	1	354869	11	NULL	NULL	NULL	NULL	mesh-like layer	CellComponent		is formed					bacteria	Organism	ouside;;plasma membrane of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Peptidoglycan, also known as murein, is a polymer consisting of sugars and amino acids that forms a mesh-like layer outside the plasma membrane of bacteria (but not Archaea), forming the cell wall	topic_mrs
75213	2	354869	11	NULL	NULL	0	NULL	Peptidoglycan	Chemical		is a synonym of					 murein	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Peptidoglycan, also known as murein, is a polymer consisting of sugars and amino acids that forms a mesh-like layer outside the plasma membrane of bacteria (but not Archaea), forming the cell wall	topic_mrs
75214	3	354869	11	NULL	NULL	0	NULL	Peptidoglycan	Chemical		is a type of 					 polymer	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Peptidoglycan, also known as murein, is a polymer consisting of sugars and amino acids that forms a mesh-like layer outside the plasma membrane of bacteria (but not Archaea), forming the cell wall	topic_mrs
75219	4	354869	11	NULL	NULL	0	NULL	Peptidoglycan	Chemical		consisting of					sugars	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Peptidoglycan, also known as murein, is a polymer consisting of sugars and amino acids that forms a mesh-like layer outside the plasma membrane of bacteria (but not Archaea), forming the cell wall	topic_mrs
75220	5	354869	11	NULL	NULL	0	NULL	Peptidoglycan	Chemical		consisting of					amino acids	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Peptidoglycan, also known as murein, is a polymer consisting of sugars and amino acids that forms a mesh-like layer outside the plasma membrane of bacteria (but not Archaea), forming the cell wall	topic_mrs
75221	6	354869	11	NULL	NULL	0	NULL	statement 4	Process		occurs along with					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Peptidoglycan, also known as murein, is a polymer consisting of sugars and amino acids that forms a mesh-like layer outside the plasma membrane of bacteria (but not Archaea), forming the cell wall	topic_mrs
75222	7	354869	11	NULL	NULL	0	NULL	statement 6	Process		forms					cell wall	CellComponent				NULL		0	NULL	NULL	NULL	NULL	NULL	Peptidoglycan, also known as murein, is a polymer consisting of sugars and amino acids that forms a mesh-like layer outside the plasma membrane of bacteria (but not Archaea), forming the cell wall	topic_mrs
75223	8	354869	11	NULL	NULL	0	NULL	mesh-like layer	CellComponent		is not formed					Archaea	Organism	ouside;;plasma membrane of			NULL		0	NULL	NULL	NULL	NULL	NULL	Peptidoglycan, also known as murein, is a polymer consisting of sugars and amino acids that forms a mesh-like layer outside the plasma membrane of bacteria (but not Archaea), forming the cell wall	topic_mrs
75019	1	354870	11	NULL	NULL	0	NULL	Meticillin-resistant S. aureus	Organism		is					 MRSA	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Meticillin-resistant S. aureus or MRSA, is resistant to virtually all available beta-lactam antimicrobials. This resistance is mediated by the chromosomally located mecA gene.	topic_mrs
75020	2	354870	11	NULL	NULL	0	NULL	Meticillin-resistant S. aureus	Organism		is resistant to					beta-lactam antimicrobials	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Meticillin-resistant S. aureus or MRSA, is resistant to virtually all available beta-lactam antimicrobials. This resistance is mediated by the chromosomally located mecA gene.	topic_mrs
75021	3	354870	11	NULL	NULL	0	NULL	statement 2	Process		is mediated by					mecA gene	GP	chromosomal			NULL		0	NULL	NULL	NULL	NULL	NULL	Meticillin-resistant S. aureus or MRSA, is resistant to virtually all available beta-lactam antimicrobials. This resistance is mediated by the chromosomally located mecA gene.	topic_mrs
75022	1	354871	11	NULL	NULL	0	NULL	CC398	Organism		is a lineage of					MRSA	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	CC398 is the MRSA lineage most often associated with asymptomatic carriage in intensively reared food-producing animals.	topic_mrs
75215	2	354871	11	NULL	NULL	0	NULL	statement 1	Organism		is associated with					asymptomatic carriage	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	CC398 is the MRSA lineage most often associated with asymptomatic carriage in intensively reared food-producing animals.	topic_mrs
75216	3	354871	11	NULL	NULL	0	NULL	statement 2	Process		occurs in					food-producing animals	Organism	intensively reared			NULL		0	NULL	NULL	NULL	NULL	NULL	CC398 is the MRSA lineage most often associated with asymptomatic carriage in intensively reared food-producing animals.	topic_mrs
76341	1	354874	11	NULL	NULL	0	NULL	Healthcare-acquired methicillin-resistant Staphylococcus aureus	Organism		is					HA-MRSA	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Healthcare-acquired methicillin-resistant Staphylococcus aureus, or HA-MRSA, is a potentially deadly strain of Staph aureus that is resistant to several antibiotics. 	topic_mrs
76342	2	354874	11	NULL	NULL	0	NULL	HA-MRSA	Organism		is resistant to					antibiotics		several 			NULL		0	NULL	NULL	NULL	NULL	NULL	Healthcare-acquired methicillin-resistant Staphylococcus aureus, or HA-MRSA, is a potentially deadly strain of Staph aureus that is resistant to several antibiotics. 	topic_mrs
76343	1	354875	11	NULL	NULL	0	NULL	Staphylococcus aureus	Organism		is also known as					staph	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Staphylococcus aureus (staph) is a type of bacteria 	topic_mrs
76344	2	354875	11	NULL	NULL	0	NULL	Staphylococcus aureus	Organism		is a type of 					bacteria	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Staphylococcus aureus (staph) is a type of bacteria 	topic_mrs
75234	1	354876	11	NULL	NULL	0	NULL	MRSA	Organism		is a strain of					Staphylococcus aureus bacteria	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA is, by definition, any strain of Staphylococcus aureus bacteria that has developed resistance to beta-lactam antibiotics which include the penicillins (methicillin, dicloxacillin, nafcillin, oxacillin, etc.) and the cephalosporins.	topic_mrs
75236	2	354876	11	NULL	NULL	0	NULL	statement 1	Organism		has resistance to					beta-lactam antibiotics					NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA is, by definition, any strain of Staphylococcus aureus bacteria that has developed resistance to beta-lactam antibiotics which include the penicillins (methicillin, dicloxacillin, nafcillin, oxacillin, etc.) and the cephalosporins.	topic_mrs
75237	3	354876	11	NULL	NULL	NULL	NULL	methicillin	Chemical		is a type of 					penicillin	Chemical				NULL		NULL	NULL	NULL	NULL	NULL	NULL	MRSA is, by definition, any strain of Staphylococcus aureus bacteria that has developed resistance to beta-lactam antibiotics which include the penicillins (methicillin, dicloxacillin, nafcillin, oxacillin, etc.) and the cephalosporins.	topic_mrs
75238	4	354876	11	NULL	NULL	NULL	NULL	dicloxacillin	Chemical		is a type of 					penicillin	Chemical				NULL		NULL	NULL	NULL	NULL	NULL	NULL	MRSA is, by definition, any strain of Staphylococcus aureus bacteria that has developed resistance to beta-lactam antibiotics which include the penicillins (methicillin, dicloxacillin, nafcillin, oxacillin, etc.) and the cephalosporins.	topic_mrs
75285	5	354876	11	NULL	NULL	0	NULL	nafcillin	Chemical		is a type of 					penicillin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA is, by definition, any strain of Staphylococcus aureus bacteria that has developed resistance to beta-lactam antibiotics which include the penicillins (methicillin, dicloxacillin, nafcillin, oxacillin, etc.) and the cephalosporins.	topic_mrs
75286	6	354876	11	NULL	NULL	0	NULL	oxacillin	Chemical		is a type of 					penicillin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA is, by definition, any strain of Staphylococcus aureus bacteria that has developed resistance to beta-lactam antibiotics which include the penicillins (methicillin, dicloxacillin, nafcillin, oxacillin, etc.) and the cephalosporins.	topic_mrs
75289	7	354876	11	NULL	NULL	0	NULL	penicillins	Chemical		are a group of					beta-lactam antibiotics	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA is, by definition, any strain of Staphylococcus aureus bacteria that has developed resistance to beta-lactam antibiotics which include the penicillins (methicillin, dicloxacillin, nafcillin, oxacillin, etc.) and the cephalosporins.	topic_mrs
75290	8	354876	11	NULL	NULL	0	NULL	cephalosporins	Chemical		are a group of					beta-lactam antibiotics	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA is, by definition, any strain of Staphylococcus aureus bacteria that has developed resistance to beta-lactam antibiotics which include the penicillins (methicillin, dicloxacillin, nafcillin, oxacillin, etc.) and the cephalosporins.	topic_mrs
75294	9	354876	11	NULL	NULL	0	NULL	MRSA	Organism		has resistance to					methicillin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA is, by definition, any strain of Staphylococcus aureus bacteria that has developed resistance to beta-lactam antibiotics which include the penicillins (methicillin, dicloxacillin, nafcillin, oxacillin, etc.) and the cephalosporins.	topic_mrs
75296	10	354876	11	NULL	NULL	0	NULL	MRSA	Organism		has resistance to					dicloxacillin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA is, by definition, any strain of Staphylococcus aureus bacteria that has developed resistance to beta-lactam antibiotics which include the penicillins (methicillin, dicloxacillin, nafcillin, oxacillin, etc.) and the cephalosporins.	topic_mrs
75297	11	354876	11	NULL	NULL	0	NULL	MRSA	Organism		has resistance to					nafcillin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA is, by definition, any strain of Staphylococcus aureus bacteria that has developed resistance to beta-lactam antibiotics which include the penicillins (methicillin, dicloxacillin, nafcillin, oxacillin, etc.) and the cephalosporins.	topic_mrs
75298	12	354876	11	NULL	NULL	0	NULL	MRSA	Organism		has resistance to					oxacillin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA is, by definition, any strain of Staphylococcus aureus bacteria that has developed resistance to beta-lactam antibiotics which include the penicillins (methicillin, dicloxacillin, nafcillin, oxacillin, etc.) and the cephalosporins.	topic_mrs
75302	13	354876	11	NULL	NULL	0	NULL	MRSA	Organism		has resistance to					cephalosporins	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA is, by definition, any strain of Staphylococcus aureus bacteria that has developed resistance to beta-lactam antibiotics which include the penicillins (methicillin, dicloxacillin, nafcillin, oxacillin, etc.) and the cephalosporins.	topic_mrs
75303	1	354877	11	NULL	NULL	0	NULL	vanH gene	GP		code for					protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The vanH, vanA, and vanX genes code for proteins that are necessary for the expression of resistance	topic_mrs
75304	2	354877	11	NULL	NULL	0	NULL	vanA gene	GP		code for					proteins	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The vanH, vanA, and vanX genes code for proteins that are necessary for the expression of resistance	topic_mrs
75305	3	354877	11	NULL	NULL	0	NULL	vanX gene	GP		code for					protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The vanH, vanA, and vanX genes code for proteins that are necessary for the expression of resistance	topic_mrs
75306	4	354877	11	NULL	NULL	0	NULL	statement 1	GP		express					resistance	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The vanH, vanA, and vanX genes code for proteins that are necessary for the expression of resistance	topic_mrs
75307	5	354877	11	NULL	NULL	0	NULL	statement 2	GP		express					resistance	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The vanH, vanA, and vanX genes code for proteins that are necessary for the expression of resistance	topic_mrs
75308	6	354877	11	NULL	NULL	0	NULL	statement 3	GP		express					resistance	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The vanH, vanA, and vanX genes code for proteins that are necessary for the expression of resistance	topic_mrs
75309	1	354878	11	NULL	NULL	0	NULL	VanA-type resistance	Process		is inducible resistance to		high-level			vancomycin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	VanA-type resistance is characterized by high-level inducible resistance to both vancomycin and teicoplanin	topic_mrs
75310	2	354878	11	NULL	NULL	0	NULL	VanA-type resistance	Process		is inducible resistance to		high-level			teicoplanin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	VanA-type resistance is characterized by high-level inducible resistance to both vancomycin and teicoplanin	topic_mrs
75311	1	354879	11	NULL	NULL	0	NULL	Mupirocin	Chemical		is a type of 					antibiotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Mupirocin (Bactroban or Centany) is an antibiotic originally isolated from Pseudomonas fluorescens	topic_mrs
75312	2	354879	11	NULL	NULL	0	NULL	Mupirocin	Chemical		is also known as					Bactroban	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Mupirocin (Bactroban or Centany) is an antibiotic originally isolated from Pseudomonas fluorescens	topic_mrs
75313	3	354879	11	NULL	NULL	0	NULL	Mupirocin	Chemical		is also known as					Centany	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Mupirocin (Bactroban or Centany) is an antibiotic originally isolated from Pseudomonas fluorescens	topic_mrs
75314	4	354879	11	NULL	NULL	0	NULL	Mupirocin	Chemical		isolates from					Pseudomonas fluorescens	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Mupirocin (Bactroban or Centany) is an antibiotic originally isolated from Pseudomonas fluorescens	topic_mrs
73937	1	354881	5	NULL	NULL	0	NULL	drugs	Chemical		dose not cure					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Drugs don't cure autism, but many autistic suffer from multiple problems such as depression or seizures, and the drugs can help with those secondary problems.	topic_aut
73938	2	354881	5	NULL	NULL	0	NULL	autistic	GroupOfPeople		suffer from					depression	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Drugs don't cure autism, but many autistic suffer from multiple problems such as depression or seizures, and the drugs can help with those secondary problems.	topic_aut
73939	3	354881	5	NULL	NULL	0	NULL	autistic	GroupOfPeople		suffer from					seizures	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Drugs don't cure autism, but many autistic suffer from multiple problems such as depression or seizures, and the drugs can help with those secondary problems.	topic_aut
75315	1	354881	5	11	NULL	0	NULL	depression	MedicalFinding		is a secondary problem of					 autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Drugs don't cure autism, but many autistic suffer from multiple problems such as depression or seizures, and the drugs can help with those secondary problems.	topic_aut
75316	1	354881	5	11	NULL	0	NULL	seizures	MedicalFinding		is a secondary problem of					 autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Drugs don't cure autism, but many autistic suffer from multiple problems such as depression or seizures, and the drugs can help with those secondary problems.	topic_aut
73940	1	354882	5	NULL	NULL	0	NULL	Mellaril	Chemical		is a type of					antipsychotics	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Anti psychotics (Mellaril, Haldol, Thorazine) - used to treat severe aggression, self-injurous behavior, agitation or insomnia	topic_aut
73941	2	354882	5	NULL	NULL	0	NULL	Haldol	Chemical		is a type of					antipsychotics	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Anti psychotics (Mellaril, Haldol, Thorazine) - used to treat severe aggression, self-injurous behavior, agitation or insomnia	topic_aut
73942	3	354882	5	NULL	NULL	0	NULL	Thorazine	Chemical		is a type of					antipsychotics	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Anti psychotics (Mellaril, Haldol, Thorazine) - used to treat severe aggression, self-injurous behavior, agitation or insomnia	topic_aut
73943	4	354882	5	NULL	NULL	0	NULL	aggression	MedicalFinding	severe	is treated with					Mellaril	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Anti psychotics (Mellaril, Haldol, Thorazine) - used to treat severe aggression, self-injurous behavior, agitation or insomnia	topic_aut
73944	5	354882	5	NULL	NULL	0	NULL	aggression	MedicalFinding	severe	is treated with					Haldol	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Anti psychotics (Mellaril, Haldol, Thorazine) - used to treat severe aggression, self-injurous behavior, agitation or insomnia	topic_aut
73945	6	354882	5	NULL	NULL	0	NULL	aggression	MedicalFinding	severe	is treated with					Thorazine	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Anti psychotics (Mellaril, Haldol, Thorazine) - used to treat severe aggression, self-injurous behavior, agitation or insomnia	topic_aut
73946	7	354882	5	NULL	NULL	0	NULL	self-injurous behavior	MedicalFinding		is treated with					Mellaril	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Anti psychotics (Mellaril, Haldol, Thorazine) - used to treat severe aggression, self-injurous behavior, agitation or insomnia	topic_aut
73947	8	354882	5	NULL	NULL	0	NULL	self-injurous behavior	MedicalFinding		is treated with					Haldol	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Anti psychotics (Mellaril, Haldol, Thorazine) - used to treat severe aggression, self-injurous behavior, agitation or insomnia	topic_aut
73948	9	354882	5	NULL	NULL	0	NULL	self-injurous behavior	MedicalFinding		is treated with					Thorazine	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Anti psychotics (Mellaril, Haldol, Thorazine) - used to treat severe aggression, self-injurous behavior, agitation or insomnia	topic_aut
73949	10	354882	5	NULL	NULL	0	NULL	agitation	MedicalFinding		is treated with					Mellaril	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Anti psychotics (Mellaril, Haldol, Thorazine) - used to treat severe aggression, self-injurous behavior, agitation or insomnia	topic_aut
73950	11	354882	5	NULL	NULL	0	NULL	agitation	MedicalFinding		is treated with					Haldol	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Anti psychotics (Mellaril, Haldol, Thorazine) - used to treat severe aggression, self-injurous behavior, agitation or insomnia	topic_aut
73951	12	354882	5	NULL	NULL	0	NULL	agitation	MedicalFinding		is treated with					Thorazine	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Anti psychotics (Mellaril, Haldol, Thorazine) - used to treat severe aggression, self-injurous behavior, agitation or insomnia	topic_aut
73952	13	354882	5	NULL	NULL	0	NULL	insomnia	MedicalFinding		is treated with					Mellaril	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Anti psychotics (Mellaril, Haldol, Thorazine) - used to treat severe aggression, self-injurous behavior, agitation or insomnia	topic_aut
73953	14	354882	5	NULL	NULL	0	NULL	insomnia	MedicalFinding		is treated with					Haldol	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Anti psychotics (Mellaril, Haldol, Thorazine) - used to treat severe aggression, self-injurous behavior, agitation or insomnia	topic_aut
73954	15	354882	5	NULL	NULL	0	NULL	insomnia	MedicalFinding		is treated with					Thorazine	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Anti psychotics (Mellaril, Haldol, Thorazine) - used to treat severe aggression, self-injurous behavior, agitation or insomnia	topic_aut
73955	1	354883	5	NULL	NULL	0	NULL	Tegretol	Chemical		is a type of					Anticonvulsants 	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Anticonvulsants (Tegretol, Depakote, Dilantin) - used to control seizures	topic_aut
73956	2	354883	5	NULL	NULL	0	NULL	Depakote	Chemical		is a type of					Anticonvulsants	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Anticonvulsants (Tegretol, Depakote, Dilantin) - used to control seizures	topic_aut
73957	3	354883	5	NULL	NULL	0	NULL	Dilantin	Chemical		is a type of					Anticonvulsants	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Anticonvulsants (Tegretol, Depakote, Dilantin) - used to control seizures	topic_aut
73958	4	354883	5	NULL	NULL	0	NULL	seizures	MedicalFinding		is controlled by					Tegretol	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Anticonvulsants (Tegretol, Depakote, Dilantin) - used to control seizures	topic_aut
73959	5	354883	5	NULL	NULL	0	NULL	seizures	MedicalFinding		is controlled by					Depakote	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Anticonvulsants (Tegretol, Depakote, Dilantin) - used to control seizures	topic_aut
73960	6	354883	5	NULL	NULL	0	NULL	seizures	MedicalFinding		is controlled by					Dilantin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Anticonvulsants (Tegretol, Depakote, Dilantin) - used to control seizures	topic_aut
73961	1	354884	5	NULL	NULL	0	NULL	Lithium	Chemical		is a type of					anti depressant	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Anti depression (Lithium, Depakote) - used for bipolar manic depression	topic_aut
73962	2	354884	5	NULL	NULL	0	NULL	Depakote	Chemical		is a type of					anti depressant	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Anti depression (Lithium, Depakote) - used for bipolar manic depression	topic_aut
73963	3	354884	5	NULL	NULL	0	NULL	bipolar manic depression	MedicalFinding		is treated with					Lithium	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Anti depression (Lithium, Depakote) - used for bipolar manic depression	topic_aut
73964	4	354884	5	NULL	NULL	0	NULL	bipolar manic depression	MedicalFinding		is treated with					Depakote	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Anti depression (Lithium, Depakote) - used for bipolar manic depression	topic_aut
73965	1	354885	5	NULL	NULL	0	NULL	Valium	Chemical		is a type of					Anti anxiety drug	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Anti anxiety (Valium, Librium) 	topic_aut
73966	2	354885	5	NULL	NULL	0	NULL	Librium	Chemical		is a type of					Anti anxiety drug	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Anti anxiety (Valium, Librium) 	topic_aut
73967	1	354886	5	NULL	NULL	0	NULL	Nadolol	Chemical		is a type of					beta blocker	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Beta Blockers (Nadolol, Buspirone)-used to decrease aggression or hyperactivity	topic_aut
73968	2	354886	5	NULL	NULL	0	NULL	Buspirone	Chemical		is a type of					beta blocker	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Beta Blockers (Nadolol, Buspirone)-used to decrease aggression or hyperactivity	topic_aut
73969	3	354886	5	NULL	NULL	0	NULL	Nadolol	Chemical		decreases					aggression	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Beta Blockers (Nadolol, Buspirone)-used to decrease aggression or hyperactivity	topic_aut
73970	4	354886	5	NULL	NULL	0	NULL	Nadolol	Chemical		decreases					hyperactivity	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Beta Blockers (Nadolol, Buspirone)-used to decrease aggression or hyperactivity	topic_aut
73971	5	354886	5	NULL	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Beta Blockers (Nadolol, Buspirone)-used to decrease aggression or hyperactivity	topic_aut
73972	6	354886	5	NULL	NULL	0	NULL	Buspirone	Chemical		decreases					aggression	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Beta Blockers (Nadolol, Buspirone)-used to decrease aggression or hyperactivity	topic_aut
73973	7	354886	5	NULL	NULL	0	NULL	Buspirone	Chemical		decreases					hyperactivity	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Beta Blockers (Nadolol, Buspirone)-used to decrease aggression or hyperactivity	topic_aut
73974	8	354886	5	NULL	NULL	0	NULL	statement 6	Process		is an alternative to					statement 7	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Beta Blockers (Nadolol, Buspirone)-used to decrease aggression or hyperactivity	topic_aut
73975	1	354887	5	NULL	NULL	NULL	NULL	Naltrexone/Trexan	Chemical		is a type of					opiate blocker	Chemical				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Opiate Blockers (Naltrexone/Trexan) - control self injurious behaviors	topic_aut
73976	2	354887	5	NULL	NULL	NULL	NULL	Naltrexone/Trexan	Chemical		controls					self injurious behaviors	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Opiate Blockers (Naltrexone/Trexan) - control self injurious behaviors	topic_aut
73977	1	354888	5	NULL	NULL	0	NULL	Chloral Hydrate	Chemical		is a type of					sedative	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Sedatives (Chloral Hydrate, Noctec, and Benadryl) - for difficulty sleeping	topic_aut
73978	2	354888	5	NULL	NULL	0	NULL	Noctec	Chemical		is a type of					sedative	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Sedatives (Chloral Hydrate, Noctec, and Benadryl) - for difficulty sleeping	topic_aut
73979	3	354888	5	NULL	NULL	0	NULL	Benadryl	Chemical		is a type of					sedative	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Sedatives (Chloral Hydrate, Noctec, and Benadryl) - for difficulty sleeping	topic_aut
73980	4	354888	5	NULL	NULL	0	NULL	Chloral Hydrate	Chemical		treats					sleeping difficulty	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Sedatives (Chloral Hydrate, Noctec, and Benadryl) - for difficulty sleeping	topic_aut
73981	5	354888	5	NULL	NULL	0	NULL	Noctec	Chemical		treats					sleeping difficulty	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Sedatives (Chloral Hydrate, Noctec, and Benadryl) - for difficulty sleeping	topic_aut
73982	6	354888	5	NULL	NULL	0	NULL	Benadryl	Chemical		treats					sleeping difficulty	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Sedatives (Chloral Hydrate, Noctec, and Benadryl) - for difficulty sleeping	topic_aut
73983	1	354889	5	NULL	NULL	0	NULL	Ritalin	Chemical		is a type of					stimulant	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulants (Ritalin, Dexedrine)-for hyperactivity and attention or concentration problems	topic_aut
73984	2	354889	5	NULL	NULL	0	NULL	Dexedrine	Chemical		is a type of					stimulant	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulants (Ritalin, Dexedrine)-for hyperactivity and attention or concentration problems	topic_aut
73985	3	354889	5	NULL	NULL	0	NULL	hyperactivity	MedicalFinding		is treated with					Ritalin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulants (Ritalin, Dexedrine)-for hyperactivity and attention or concentration problems	topic_aut
73986	4	354889	5	NULL	NULL	0	NULL	hyperactivity	MedicalFinding		is treated with					Dexedrine	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulants (Ritalin, Dexedrine)-for hyperactivity and attention or concentration problems	topic_aut
73987	5	354889	5	NULL	NULL	0	NULL	attention or concentration problems	MedicalFinding		is treated with					Ritalin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulants (Ritalin, Dexedrine)-for hyperactivity and attention or concentration problems	topic_aut
73988	6	354889	5	NULL	NULL	0	NULL	attention or concentration problems	MedicalFinding		is treated with					Dexedrine	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulants (Ritalin, Dexedrine)-for hyperactivity and attention or concentration problems	topic_aut
74072	1	354890	5	NULL	NULL	0	NULL	candida albicans	Organism		is a synonym of					yeast	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	There are some evidence that candida albicans (yeast) may cause or exacerbate behavior and health problems in autistic individuals. The only physical symptoms are vaginal yeast infections and thrush (white patches in mouth). Candida overgrowth is often attributed to long term antibiotic treatments. It has been reported that some children whose autistic tendencies surfaced at 18- 24 months had been continuously treated with antibiotics to control chronic ear infections. The treatment doesn't cure autism, but is helpful for some autistic children.	topic_aut
74073	2	354890	5	NULL	NULL	0	NULL	candida albicans	Organism		cause		may			behavior problems	MedicalFinding				NULL	autistic individulas	0	NULL	NULL	NULL	NULL	NULL	There are some evidence that candida albicans (yeast) may cause or exacerbate behavior and health problems in autistic individuals. The only physical symptoms are vaginal yeast infections and thrush (white patches in mouth). Candida overgrowth is often attributed to long term antibiotic treatments. It has been reported that some children whose autistic tendencies surfaced at 18- 24 months had been continuously treated with antibiotics to control chronic ear infections. The treatment doesn't cure autism, but is helpful for some autistic children.	topic_aut
74074	3	354890	5	NULL	NULL	0	NULL	candida albicans	Organism		cause		may			health problems	MedicalFinding				NULL	autistic individulas	0	NULL	NULL	NULL	NULL	NULL	There are some evidence that candida albicans (yeast) may cause or exacerbate behavior and health problems in autistic individuals. The only physical symptoms are vaginal yeast infections and thrush (white patches in mouth). Candida overgrowth is often attributed to long term antibiotic treatments. It has been reported that some children whose autistic tendencies surfaced at 18- 24 months had been continuously treated with antibiotics to control chronic ear infections. The treatment doesn't cure autism, but is helpful for some autistic children.	topic_aut
74075	4	354890	5	NULL	NULL	0	NULL	vagina	OrganismPart	infection of	is a symptom of		physical			candida outgrowth	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	There are some evidence that candida albicans (yeast) may cause or exacerbate behavior and health problems in autistic individuals. The only physical symptoms are vaginal yeast infections and thrush (white patches in mouth). Candida overgrowth is often attributed to long term antibiotic treatments. It has been reported that some children whose autistic tendencies surfaced at 18- 24 months had been continuously treated with antibiotics to control chronic ear infections. The treatment doesn't cure autism, but is helpful for some autistic children.	topic_aut
74076	5	354890	5	NULL	NULL	0	NULL	thrush	MedicalFinding		is a symptom of		physical			candida outgrowth	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	There are some evidence that candida albicans (yeast) may cause or exacerbate behavior and health problems in autistic individuals. The only physical symptoms are vaginal yeast infections and thrush (white patches in mouth). Candida overgrowth is often attributed to long term antibiotic treatments. It has been reported that some children whose autistic tendencies surfaced at 18- 24 months had been continuously treated with antibiotics to control chronic ear infections. The treatment doesn't cure autism, but is helpful for some autistic children.	topic_aut
74077	6	354890	5	NULL	NULL	0	NULL	thrush	MedicalFinding		is a type of					white patches in mouth	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	There are some evidence that candida albicans (yeast) may cause or exacerbate behavior and health problems in autistic individuals. The only physical symptoms are vaginal yeast infections and thrush (white patches in mouth). Candida overgrowth is often attributed to long term antibiotic treatments. It has been reported that some children whose autistic tendencies surfaced at 18- 24 months had been continuously treated with antibiotics to control chronic ear infections. The treatment doesn't cure autism, but is helpful for some autistic children.	topic_aut
74082	1	354892	5	NULL	NULL	0	NULL	autistic individuals	GroupOfPeople		experience					sensory dysfunction	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Auditory training can be considered a form of sensory integration in which stimulation  may sensitize or desensitize one or more senses. Theoretically speaking, if one or more  senses are impaired in an individual, he or she may develop a distorted perception of the   environment. There has been much research in the past 15 years to indicate that many  autistic individuals have sensory dysfunction in one or more areas	topic_aut
74083	2	354892	5	NULL	NULL	0	NULL	senses	PhysicalPhenomenon	impaired	develops					environment	PhysicalPhenomenon	distorted perception of			NULL		0	NULL	NULL	NULL	NULL	NULL	Auditory training can be considered a form of sensory integration in which stimulation  may sensitize or desensitize one or more senses. Theoretically speaking, if one or more  senses are impaired in an individual, he or she may develop a distorted perception of the   environment. There has been much research in the past 15 years to indicate that many  autistic individuals have sensory dysfunction in one or more areas	topic_aut
76345	1	354894	11	NULL	NULL	0	NULL	antibacterial	Chemical		kills					bacteria	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	An antibacterial is a substance that kills bacteria or slows their growth. The term 'antibiotic' was coined by Selman Waksman in 1942 to describe any substance produced by a microorganism that is antagonistic to the growth of other microorganisms in high dilution.	topic_mrs
76346	2	354894	11	NULL	NULL	0	NULL	antibacterial	Chemical		slows					Bacterial growth	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	An antibacterial is a substance that kills bacteria or slows their growth. The term 'antibiotic' was coined by Selman Waksman in 1942 to describe any substance produced by a microorganism that is antagonistic to the growth of other microorganisms in high dilution.	topic_mrs
76347	3	354894	11	NULL	NULL	0	NULL	statement 1	Process		is an alternative to 					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	An antibacterial is a substance that kills bacteria or slows their growth. The term 'antibiotic' was coined by Selman Waksman in 1942 to describe any substance produced by a microorganism that is antagonistic to the growth of other microorganisms in high dilution.	topic_mrs
75408	1	354895	11	NULL	NULL	0	NULL	Bactroban	Chemical		contains					mupirocin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Bactroban contains mupirocin, an antibiotic. Mupirocin prevents bacteria from growing on your skin.	topic_mrs
75409	2	354895	11	NULL	NULL	0	NULL	mupirocin	Chemical		is a type of 					antibiotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Bactroban contains mupirocin, an antibiotic. Mupirocin prevents bacteria from growing on your skin.	topic_mrs
75410	3	354895	11	NULL	NULL	0	NULL	Mupirocin	Chemical		prevents					Bacterial growth	Process	skin			NULL		0	NULL	NULL	NULL	NULL	NULL	Bactroban contains mupirocin, an antibiotic. Mupirocin prevents bacteria from growing on your skin.	topic_mrs
75411	1	354896	11	NULL	NULL	0	NULL	Mupirocin	Chemical		is a type of 					antibiotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Mupirocin  is an antibiotic originally isolated from Pseudomonas fluorescens 	topic_mrs
75412	2	354896	11	NULL	NULL	0	NULL	Mupirocin	Chemical		isolated from					Pseudomonas fluorescens	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Mupirocin  is an antibiotic originally isolated from Pseudomonas fluorescens 	topic_mrs
74278	1	354897	7	NULL	NULL	0	NULL	HNPCC	MedicalFinding		is a type of					genetically heterogeneous disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Hereditary non-polyposis colorectal cancer (HNPCC or Lynch syndrome), is a genetically heterogeneous disorder that is believed to account for 2-10 per cent of all the colorectal cancer cases. The disease follows autosomal dominant inheritance pattern with high penetrance (85%) and younger age of onset when compared to patients with sporadic tumours.	topic_ccc
74279	2	354897	7	NULL	NULL	0	NULL	HNPCC	MedicalFinding		is 					Lynch syndrome	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Hereditary non-polyposis colorectal cancer (HNPCC or Lynch syndrome), is a genetically heterogeneous disorder that is believed to account for 2-10 per cent of all the colorectal cancer cases. The disease follows autosomal dominant inheritance pattern with high penetrance (85%) and younger age of onset when compared to patients with sporadic tumours.	topic_ccc
74280	3	354897	7	NULL	NULL	0	NULL	HNPCC	MedicalFinding		is					Hereditary non-polyposis colorectal cancer					NULL		0	NULL	NULL	NULL	NULL	NULL	Hereditary non-polyposis colorectal cancer (HNPCC or Lynch syndrome), is a genetically heterogeneous disorder that is believed to account for 2-10 per cent of all the colorectal cancer cases. The disease follows autosomal dominant inheritance pattern with high penetrance (85%) and younger age of onset when compared to patients with sporadic tumours.	topic_ccc
74281	4	354897	7	NULL	NULL	0	NULL	HNPCC	MedicalFinding		follows					autosomal dominant inheritance pattern	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Hereditary non-polyposis colorectal cancer (HNPCC or Lynch syndrome), is a genetically heterogeneous disorder that is believed to account for 2-10 per cent of all the colorectal cancer cases. The disease follows autosomal dominant inheritance pattern with high penetrance (85%) and younger age of onset when compared to patients with sporadic tumours.	topic_ccc
74282	1	354899	7	NULL	NULL	0	NULL	colorectal cancer	MedicalFinding		predisposition with		genetic			autosomal dominant of pattern of inheritance	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	1-5% of all patients presenting with colorectal cancer, have an underlying genetic predisposition with an autosomal dominant of pattern of inheritance. However, endometrial cancer, stomach cancer, small bowel cancer, urinary tract cancer and skin cancer among others are also inherent to the syndrome.	topic_ccc
74283	1	354900	7	NULL	NULL	0	NULL	hMSH2 genes	GP		located at					chromosome 2p21	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	The genomic loci for the mismatch repair genes hMSH2 and hMSH6 were mapped by fluorescence in situ hybridization, analysis of radiation hybrid panel markers, and linkage analysis of syntenic chromosome regions between human and mouse. Both genes were localized to chromosome 2p21	topic_ccc
74284	2	354900	7	NULL	NULL	0	NULL	hMSH6 genes	GP		located at					chromosome 2p21	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	The genomic loci for the mismatch repair genes hMSH2 and hMSH6 were mapped by fluorescence in situ hybridization, analysis of radiation hybrid panel markers, and linkage analysis of syntenic chromosome regions between human and mouse. Both genes were localized to chromosome 2p21	topic_ccc
74285	1	354902	7	NULL	NULL	0	NULL	VEGF	GP		expressed in					metastatic neoplasm	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the correlation between expression of vascular endothelial growth factor (VEGF), basic fibroblast growth factor (bFGF), and their receptors with vascularity, metastasis, and proliferative index of human colon cancers.Expression of VEGF and KDR was higher in metastatic than in nonmetastatic neoplasms and directly correlated with the extent of neovascularization and the degree of proliferation, whereas expression of bFGF, flt-1, bek, and flg did not differ among tumor types. Vessel counts were greater in metastatic tumors than in nonmetastatic tumors.	topic_ccc
74286	2	354902	7	NULL	NULL	0	NULL	VEGF	GP		expressed in					nonmetastatic neoplasm	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the correlation between expression of vascular endothelial growth factor (VEGF), basic fibroblast growth factor (bFGF), and their receptors with vascularity, metastasis, and proliferative index of human colon cancers.Expression of VEGF and KDR was higher in metastatic than in nonmetastatic neoplasms and directly correlated with the extent of neovascularization and the degree of proliferation, whereas expression of bFGF, flt-1, bek, and flg did not differ among tumor types. Vessel counts were greater in metastatic tumors than in nonmetastatic tumors.	topic_ccc
74287	3	354902	7	NULL	NULL	0	NULL	statement 1	Process		is higher than					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the correlation between expression of vascular endothelial growth factor (VEGF), basic fibroblast growth factor (bFGF), and their receptors with vascularity, metastasis, and proliferative index of human colon cancers.Expression of VEGF and KDR was higher in metastatic than in nonmetastatic neoplasms and directly correlated with the extent of neovascularization and the degree of proliferation, whereas expression of bFGF, flt-1, bek, and flg did not differ among tumor types. Vessel counts were greater in metastatic tumors than in nonmetastatic tumors.	topic_ccc
74288	4	354902	7	NULL	NULL	0	NULL	KDR	GP		expressed in					metastatic neoplasm	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the correlation between expression of vascular endothelial growth factor (VEGF), basic fibroblast growth factor (bFGF), and their receptors with vascularity, metastasis, and proliferative index of human colon cancers.Expression of VEGF and KDR was higher in metastatic than in nonmetastatic neoplasms and directly correlated with the extent of neovascularization and the degree of proliferation, whereas expression of bFGF, flt-1, bek, and flg did not differ among tumor types. Vessel counts were greater in metastatic tumors than in nonmetastatic tumors.	topic_ccc
74289	5	354902	7	NULL	NULL	0	NULL	KDR	GP		expressed in					nonmetastatic neoplasm	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the correlation between expression of vascular endothelial growth factor (VEGF), basic fibroblast growth factor (bFGF), and their receptors with vascularity, metastasis, and proliferative index of human colon cancers.Expression of VEGF and KDR was higher in metastatic than in nonmetastatic neoplasms and directly correlated with the extent of neovascularization and the degree of proliferation, whereas expression of bFGF, flt-1, bek, and flg did not differ among tumor types. Vessel counts were greater in metastatic tumors than in nonmetastatic tumors.	topic_ccc
74290	6	354902	7	NULL	NULL	0	NULL	statement 4	Process		is higher than					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the correlation between expression of vascular endothelial growth factor (VEGF), basic fibroblast growth factor (bFGF), and their receptors with vascularity, metastasis, and proliferative index of human colon cancers.Expression of VEGF and KDR was higher in metastatic than in nonmetastatic neoplasms and directly correlated with the extent of neovascularization and the degree of proliferation, whereas expression of bFGF, flt-1, bek, and flg did not differ among tumor types. Vessel counts were greater in metastatic tumors than in nonmetastatic tumors.	topic_ccc
74291	7	354902	7	NULL	NULL	0	NULL	statement 3	Process		correlates with					neovascularization	Process	extent of			NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the correlation between expression of vascular endothelial growth factor (VEGF), basic fibroblast growth factor (bFGF), and their receptors with vascularity, metastasis, and proliferative index of human colon cancers.Expression of VEGF and KDR was higher in metastatic than in nonmetastatic neoplasms and directly correlated with the extent of neovascularization and the degree of proliferation, whereas expression of bFGF, flt-1, bek, and flg did not differ among tumor types. Vessel counts were greater in metastatic tumors than in nonmetastatic tumors.	topic_ccc
74292	8	354902	7	NULL	NULL	0	NULL	statement 6	Process		correlates with					neovascularization	Process	extent of			NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the correlation between expression of vascular endothelial growth factor (VEGF), basic fibroblast growth factor (bFGF), and their receptors with vascularity, metastasis, and proliferative index of human colon cancers.Expression of VEGF and KDR was higher in metastatic than in nonmetastatic neoplasms and directly correlated with the extent of neovascularization and the degree of proliferation, whereas expression of bFGF, flt-1, bek, and flg did not differ among tumor types. Vessel counts were greater in metastatic tumors than in nonmetastatic tumors.	topic_ccc
74293	9	354902	7	NULL	NULL	0	NULL	statement 3	Process		correlates with					proliferation	Process	degree of			NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the correlation between expression of vascular endothelial growth factor (VEGF), basic fibroblast growth factor (bFGF), and their receptors with vascularity, metastasis, and proliferative index of human colon cancers.Expression of VEGF and KDR was higher in metastatic than in nonmetastatic neoplasms and directly correlated with the extent of neovascularization and the degree of proliferation, whereas expression of bFGF, flt-1, bek, and flg did not differ among tumor types. Vessel counts were greater in metastatic tumors than in nonmetastatic tumors.	topic_ccc
74294	10	354902	7	NULL	NULL	0	NULL	statement 6	Process		correlates with					proliferation	Process	degree of			NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the correlation between expression of vascular endothelial growth factor (VEGF), basic fibroblast growth factor (bFGF), and their receptors with vascularity, metastasis, and proliferative index of human colon cancers.Expression of VEGF and KDR was higher in metastatic than in nonmetastatic neoplasms and directly correlated with the extent of neovascularization and the degree of proliferation, whereas expression of bFGF, flt-1, bek, and flg did not differ among tumor types. Vessel counts were greater in metastatic tumors than in nonmetastatic tumors.	topic_ccc
74295	11	354902	7	NULL	NULL	0	NULL	bFGF	GP	expression of	does not differ among					tumor types	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the correlation between expression of vascular endothelial growth factor (VEGF), basic fibroblast growth factor (bFGF), and their receptors with vascularity, metastasis, and proliferative index of human colon cancers.Expression of VEGF and KDR was higher in metastatic than in nonmetastatic neoplasms and directly correlated with the extent of neovascularization and the degree of proliferation, whereas expression of bFGF, flt-1, bek, and flg did not differ among tumor types. Vessel counts were greater in metastatic tumors than in nonmetastatic tumors.	topic_ccc
74296	12	354902	7	NULL	NULL	NULL	NULL	flt-1	GP	expression of	does not differ among					tumor types	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	We studied the correlation between expression of vascular endothelial growth factor (VEGF), basic fibroblast growth factor (bFGF), and their receptors with vascularity, metastasis, and proliferative index of human colon cancers.Expression of VEGF and KDR was higher in metastatic than in nonmetastatic neoplasms and directly correlated with the extent of neovascularization and the degree of proliferation, whereas expression of bFGF, flt-1, bek, and flg did not differ among tumor types. Vessel counts were greater in metastatic tumors than in nonmetastatic tumors.	topic_ccc
74297	13	354902	7	NULL	NULL	0	NULL	 bek	GP	expression of	does not differ among					tumor types	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the correlation between expression of vascular endothelial growth factor (VEGF), basic fibroblast growth factor (bFGF), and their receptors with vascularity, metastasis, and proliferative index of human colon cancers.Expression of VEGF and KDR was higher in metastatic than in nonmetastatic neoplasms and directly correlated with the extent of neovascularization and the degree of proliferation, whereas expression of bFGF, flt-1, bek, and flg did not differ among tumor types. Vessel counts were greater in metastatic tumors than in nonmetastatic tumors.	topic_ccc
74298	14	354902	7	NULL	NULL	0	NULL	 flg	GP	expression of	does not differ among					tumor types	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the correlation between expression of vascular endothelial growth factor (VEGF), basic fibroblast growth factor (bFGF), and their receptors with vascularity, metastasis, and proliferative index of human colon cancers.Expression of VEGF and KDR was higher in metastatic than in nonmetastatic neoplasms and directly correlated with the extent of neovascularization and the degree of proliferation, whereas expression of bFGF, flt-1, bek, and flg did not differ among tumor types. Vessel counts were greater in metastatic tumors than in nonmetastatic tumors.	topic_ccc
74299	15	354902	7	NULL	NULL	0	NULL	metastatic tumor	MedicalFinding	vessel counts in	is greater than					nonmetastatic tumors	MedicalFinding	vessel counts in			NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the correlation between expression of vascular endothelial growth factor (VEGF), basic fibroblast growth factor (bFGF), and their receptors with vascularity, metastasis, and proliferative index of human colon cancers.Expression of VEGF and KDR was higher in metastatic than in nonmetastatic neoplasms and directly correlated with the extent of neovascularization and the degree of proliferation, whereas expression of bFGF, flt-1, bek, and flg did not differ among tumor types. Vessel counts were greater in metastatic tumors than in nonmetastatic tumors.	topic_ccc
74300	16	354902	7	NULL	NULL	0	NULL	VEGF	GP		is					vascular endothelial growth factor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the correlation between expression of vascular endothelial growth factor (VEGF), basic fibroblast growth factor (bFGF), and their receptors with vascularity, metastasis, and proliferative index of human colon cancers.Expression of VEGF and KDR was higher in metastatic than in nonmetastatic neoplasms and directly correlated with the extent of neovascularization and the degree of proliferation, whereas expression of bFGF, flt-1, bek, and flg did not differ among tumor types. Vessel counts were greater in metastatic tumors than in nonmetastatic tumors.	topic_ccc
74301	17	354902	7	NULL	NULL	0	NULL	bFGF	GP		is					basic fibroblast growth factor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the correlation between expression of vascular endothelial growth factor (VEGF), basic fibroblast growth factor (bFGF), and their receptors with vascularity, metastasis, and proliferative index of human colon cancers.Expression of VEGF and KDR was higher in metastatic than in nonmetastatic neoplasms and directly correlated with the extent of neovascularization and the degree of proliferation, whereas expression of bFGF, flt-1, bek, and flg did not differ among tumor types. Vessel counts were greater in metastatic tumors than in nonmetastatic tumors.	topic_ccc
74302	1	354903	7	NULL	NULL	0	NULL	VEGF	GP		expressed in					metastatic neoplasm	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the correlation between expression of vascular endothelial growth factor (VEGF), basic fibroblast growth factor (bFGF), and their receptors with vascularity, metastasis, and proliferative index of human colon cancers.Expression of VEGF and KDR was higher in metastatic than in nonmetastatic neoplasms and directly correlated with the extent of neovascularization and the degree of proliferation	topic_ccc
74303	2	354903	7	NULL	NULL	0	NULL	VEGF	GP		expressed in					nonmetastatic neoplasm	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the correlation between expression of vascular endothelial growth factor (VEGF), basic fibroblast growth factor (bFGF), and their receptors with vascularity, metastasis, and proliferative index of human colon cancers.Expression of VEGF and KDR was higher in metastatic than in nonmetastatic neoplasms and directly correlated with the extent of neovascularization and the degree of proliferation	topic_ccc
74304	3	354903	7	NULL	NULL	0	NULL	statement 1	Process		is higher than					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the correlation between expression of vascular endothelial growth factor (VEGF), basic fibroblast growth factor (bFGF), and their receptors with vascularity, metastasis, and proliferative index of human colon cancers.Expression of VEGF and KDR was higher in metastatic than in nonmetastatic neoplasms and directly correlated with the extent of neovascularization and the degree of proliferation	topic_ccc
74305	4	354903	7	NULL	NULL	0	NULL	KDR	GP		expressed in					metastatic neoplasm	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the correlation between expression of vascular endothelial growth factor (VEGF), basic fibroblast growth factor (bFGF), and their receptors with vascularity, metastasis, and proliferative index of human colon cancers.Expression of VEGF and KDR was higher in metastatic than in nonmetastatic neoplasms and directly correlated with the extent of neovascularization and the degree of proliferation	topic_ccc
74306	5	354903	7	NULL	NULL	0	NULL	KDR	GP		expressed in					nonmetastatic neoplasm	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the correlation between expression of vascular endothelial growth factor (VEGF), basic fibroblast growth factor (bFGF), and their receptors with vascularity, metastasis, and proliferative index of human colon cancers.Expression of VEGF and KDR was higher in metastatic than in nonmetastatic neoplasms and directly correlated with the extent of neovascularization and the degree of proliferation	topic_ccc
74307	6	354903	7	NULL	NULL	NULL	NULL	statement 4	Process		is higher than					statement 5	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	We studied the correlation between expression of vascular endothelial growth factor (VEGF), basic fibroblast growth factor (bFGF), and their receptors with vascularity, metastasis, and proliferative index of human colon cancers.Expression of VEGF and KDR was higher in metastatic than in nonmetastatic neoplasms and directly correlated with the extent of neovascularization and the degree of proliferation	topic_ccc
74308	7	354903	7	NULL	NULL	0	NULL	statement 3	Process		correlates with		directly			neovascularization	Process	extent of			NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the correlation between expression of vascular endothelial growth factor (VEGF), basic fibroblast growth factor (bFGF), and their receptors with vascularity, metastasis, and proliferative index of human colon cancers.Expression of VEGF and KDR was higher in metastatic than in nonmetastatic neoplasms and directly correlated with the extent of neovascularization and the degree of proliferation	topic_ccc
74309	8	354903	7	NULL	NULL	0	NULL	statement 6	Process		correlates with		directly			neovascularization	Process	extent of			NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the correlation between expression of vascular endothelial growth factor (VEGF), basic fibroblast growth factor (bFGF), and their receptors with vascularity, metastasis, and proliferative index of human colon cancers.Expression of VEGF and KDR was higher in metastatic than in nonmetastatic neoplasms and directly correlated with the extent of neovascularization and the degree of proliferation	topic_ccc
74310	9	354903	7	NULL	NULL	0	NULL	statement 3	Process		correlates with		directly			proliferation	Process	degree of			NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the correlation between expression of vascular endothelial growth factor (VEGF), basic fibroblast growth factor (bFGF), and their receptors with vascularity, metastasis, and proliferative index of human colon cancers.Expression of VEGF and KDR was higher in metastatic than in nonmetastatic neoplasms and directly correlated with the extent of neovascularization and the degree of proliferation	topic_ccc
74311	10	354903	7	NULL	NULL	0	NULL	statement 6	Process		correlates with		directly			proliferation	Process	degree of			NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the correlation between expression of vascular endothelial growth factor (VEGF), basic fibroblast growth factor (bFGF), and their receptors with vascularity, metastasis, and proliferative index of human colon cancers.Expression of VEGF and KDR was higher in metastatic than in nonmetastatic neoplasms and directly correlated with the extent of neovascularization and the degree of proliferation	topic_ccc
74312	11	354903	7	NULL	NULL	0	NULL	VEGF	GP		is					vascular endothelial growth factor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the correlation between expression of vascular endothelial growth factor (VEGF), basic fibroblast growth factor (bFGF), and their receptors with vascularity, metastasis, and proliferative index of human colon cancers.Expression of VEGF and KDR was higher in metastatic than in nonmetastatic neoplasms and directly correlated with the extent of neovascularization and the degree of proliferation	topic_ccc
74313	12	354903	7	NULL	NULL	0	NULL	bFGF	GP		is					basic fibroblast growth factor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the correlation between expression of vascular endothelial growth factor (VEGF), basic fibroblast growth factor (bFGF), and their receptors with vascularity, metastasis, and proliferative index of human colon cancers.Expression of VEGF and KDR was higher in metastatic than in nonmetastatic neoplasms and directly correlated with the extent of neovascularization and the degree of proliferation	topic_ccc
74314	1	354905	7	NULL	NULL	0	NULL	Microsatellite instability	NucleicAcid		is associated with					patient survival	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Microsatellite instability is an important factor associated with patient survival in Chinese sporadic colorectal cancer.\t	topic_ccc
74315	2	354905	7	NULL	NULL	0	NULL	statement 1	Process		occur in					Chinese sporadic colorectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Microsatellite instability is an important factor associated with patient survival in Chinese sporadic colorectal cancer.\t	topic_ccc
74334	1	354906	7	NULL	NULL	0	NULL	VEGF	GP		is an important					angiogenic factor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	hese findings support the hypothesis that VEGF is an important angiogenic factor in primary and metastatic human colon cancer.	topic_ccc
74335	2	354906	7	NULL	NULL	0	NULL	statement 1	Process		occur in 					primary human colon cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	hese findings support the hypothesis that VEGF is an important angiogenic factor in primary and metastatic human colon cancer.	topic_ccc
74336	3	354906	7	NULL	NULL	0	NULL	statement 1	Process		occur in					metastatic human colon cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	hese findings support the hypothesis that VEGF is an important angiogenic factor in primary and metastatic human colon cancer.	topic_ccc
74438	1	354908	7	NULL	NULL	0	NULL	CIMP	PhysicalPhenomenon		characterized by					p16	GP	abnormal methylation of		multiple CpG islands	NULL		0	NULL	NULL	NULL	NULL	NULL	CpG island methylator phenotype (CIMP) in colorectal cancers is characterized by abnormal methylation of multiple CpG islands including those in several tumor suppressor genes such as p16, hMLH1, and THBS1. \t	topic_ccc
74439	2	354908	7	NULL	NULL	0	NULL	CIMP	PhysicalPhenomenon		characterized by					hMLH1	GP	abnormal methylation of		multiple CpG islands	NULL		0	NULL	NULL	NULL	NULL	NULL	CpG island methylator phenotype (CIMP) in colorectal cancers is characterized by abnormal methylation of multiple CpG islands including those in several tumor suppressor genes such as p16, hMLH1, and THBS1. \t	topic_ccc
74440	3	354908	7	NULL	NULL	NULL	NULL	CIMP	PhysicalPhenomenon		characterized by					THBS1	GP	abnormal methylation of		multiple CpG islands	NULL		NULL	NULL	NULL	NULL	NULL	NULL	CpG island methylator phenotype (CIMP) in colorectal cancers is characterized by abnormal methylation of multiple CpG islands including those in several tumor suppressor genes such as p16, hMLH1, and THBS1. \t	topic_ccc
74441	4	354908	7	NULL	NULL	0	NULL	statement 1	Process		occur in					colorectal cancers	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	CpG island methylator phenotype (CIMP) in colorectal cancers is characterized by abnormal methylation of multiple CpG islands including those in several tumor suppressor genes such as p16, hMLH1, and THBS1. \t	topic_ccc
74442	5	354908	7	NULL	NULL	0	NULL	statement 2	Process		occur in					colorectal cancers	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	CpG island methylator phenotype (CIMP) in colorectal cancers is characterized by abnormal methylation of multiple CpG islands including those in several tumor suppressor genes such as p16, hMLH1, and THBS1. \t	topic_ccc
74443	6	354908	7	NULL	NULL	0	NULL	statement 3	Process		occur in					colorectal cancers	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	CpG island methylator phenotype (CIMP) in colorectal cancers is characterized by abnormal methylation of multiple CpG islands including those in several tumor suppressor genes such as p16, hMLH1, and THBS1. \t	topic_ccc
74444	7	354908	7	NULL	NULL	0	NULL	CIMP	PhysicalPhenomenon		is					CpG island methylator phenotype	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	NULL	NULL	CpG island methylator phenotype (CIMP) in colorectal cancers is characterized by abnormal methylation of multiple CpG islands including those in several tumor suppressor genes such as p16, hMLH1, and THBS1. \t	topic_ccc
74445	8	354908	7	NULL	NULL	0	NULL	p16	GP		is a type of					tumor suppressor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	CpG island methylator phenotype (CIMP) in colorectal cancers is characterized by abnormal methylation of multiple CpG islands including those in several tumor suppressor genes such as p16, hMLH1, and THBS1. \t	topic_ccc
74446	9	354908	7	NULL	NULL	0	NULL	hMLH1	GP		is a type of					tumor suppressor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	CpG island methylator phenotype (CIMP) in colorectal cancers is characterized by abnormal methylation of multiple CpG islands including those in several tumor suppressor genes such as p16, hMLH1, and THBS1. \t	topic_ccc
74447	10	354908	7	NULL	NULL	0	NULL	THBS1	GP		is a type of					tumor suppressor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	CpG island methylator phenotype (CIMP) in colorectal cancers is characterized by abnormal methylation of multiple CpG islands including those in several tumor suppressor genes such as p16, hMLH1, and THBS1. \t	topic_ccc
74448	1	354910	7	NULL	NULL	0	NULL	Oxygen	Chemical		associated with					genomic instability	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Oxygen is further shown to be associated with genomic instability in two additional cancer models involving the APC tumor suppressor gene and chemical carcinogenesis. 	topic_ccc
74449	2	354910	7	NULL	NULL	0	NULL	statement 1	Process		occur in					cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Oxygen is further shown to be associated with genomic instability in two additional cancer models involving the APC tumor suppressor gene and chemical carcinogenesis. 	topic_ccc
74450	3	354910	7	NULL	NULL	0	NULL	statement 2	Process		involves					APC tumor suppressor gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Oxygen is further shown to be associated with genomic instability in two additional cancer models involving the APC tumor suppressor gene and chemical carcinogenesis. 	topic_ccc
74451	4	354910	7	NULL	NULL	0	NULL	statement 2	Process		involves					chemical carcinogenesis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Oxygen is further shown to be associated with genomic instability in two additional cancer models involving the APC tumor suppressor gene and chemical carcinogenesis. 	topic_ccc
74452	1	354913	7	NULL	NULL	0	NULL	MMR genes 	GP	defects in	involved in					 renal carcinogenesis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	he complete absence of both hMLH1 and hMSH2 immunohistochemical expressions was observed only in the 3 cases with a high level of MSI. This study showed that defects in MMR genes are involved in renal carcinogenesis and correlate with the occurrence of 	topic_ccc
74453	1	354914	7	NULL	NULL	0	NULL	microsatellite loci 	NucleicAcid	instability at	attributed to					mismatch repair errors	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Instability at microsatellite loci is widely attributed to mismatch repair errors due to epigenetic alterations. Using three dinucleotide markers, D3S1313, D9S171, D17S250 and two mononucleotide markers BAT25, BATRII, we evaluated MSI in 97 cases enrolled for endoscopy of upper GI tract with symptoms of dyspepsia, reflux or dysphagia. We aimed at evaluating markers that reflect instability in esophageal malignancies, examine the prevalence of MSI in cancers and other pathologies of the esophagus, and determine the methylation status of hMLH1 gene in relation to MSI. 42% (21/50) cancers and 15.4%(2/13) precancers exhibited MSI where 85.7% cancers and 50% precancers with MSI, showed a hypermethylated hMLH1 promoter.	topic_ccc
74454	2	354914	7	NULL	NULL	0	NULL	statement 1	Process		due to					epigenetic alterations	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Instability at microsatellite loci is widely attributed to mismatch repair errors due to epigenetic alterations. Using three dinucleotide markers, D3S1313, D9S171, D17S250 and two mononucleotide markers BAT25, BATRII, we evaluated MSI in 97 cases enrolled for endoscopy of upper GI tract with symptoms of dyspepsia, reflux or dysphagia. We aimed at evaluating markers that reflect instability in esophageal malignancies, examine the prevalence of MSI in cancers and other pathologies of the esophagus, and determine the methylation status of hMLH1 gene in relation to MSI. 42% (21/50) cancers and 15.4%(2/13) precancers exhibited MSI where 85.7% cancers and 50% precancers with MSI, showed a hypermethylated hMLH1 promoter.	topic_ccc
74455	3	354914	7	NULL	NULL	0	NULL	cancers	MedicalFinding		shows					MSI	NucleicAcid	prevalence of			NULL		0	NULL	NULL	NULL	NULL	NULL	Instability at microsatellite loci is widely attributed to mismatch repair errors due to epigenetic alterations. Using three dinucleotide markers, D3S1313, D9S171, D17S250 and two mononucleotide markers BAT25, BATRII, we evaluated MSI in 97 cases enrolled for endoscopy of upper GI tract with symptoms of dyspepsia, reflux or dysphagia. We aimed at evaluating markers that reflect instability in esophageal malignancies, examine the prevalence of MSI in cancers and other pathologies of the esophagus, and determine the methylation status of hMLH1 gene in relation to MSI. 42% (21/50) cancers and 15.4%(2/13) precancers exhibited MSI where 85.7% cancers and 50% precancers with MSI, showed a hypermethylated hMLH1 promoter.	topic_ccc
74456	4	354914	7	NULL	NULL	0	NULL	precancers	MedicalFinding		shows					MSI	NucleicAcid	prevalence of			NULL		0	NULL	NULL	NULL	NULL	NULL	Instability at microsatellite loci is widely attributed to mismatch repair errors due to epigenetic alterations. Using three dinucleotide markers, D3S1313, D9S171, D17S250 and two mononucleotide markers BAT25, BATRII, we evaluated MSI in 97 cases enrolled for endoscopy of upper GI tract with symptoms of dyspepsia, reflux or dysphagia. We aimed at evaluating markers that reflect instability in esophageal malignancies, examine the prevalence of MSI in cancers and other pathologies of the esophagus, and determine the methylation status of hMLH1 gene in relation to MSI. 42% (21/50) cancers and 15.4%(2/13) precancers exhibited MSI where 85.7% cancers and 50% precancers with MSI, showed a hypermethylated hMLH1 promoter.	topic_ccc
74457	5	354914	7	NULL	NULL	NULL	NULL	statement 3	Process		involves					 hMLH1 	GP	hypermethylated		promoter	NULL		NULL	NULL	NULL	NULL	NULL	NULL	Instability at microsatellite loci is widely attributed to mismatch repair errors due to epigenetic alterations. Using three dinucleotide markers, D3S1313, D9S171, D17S250 and two mononucleotide markers BAT25, BATRII, we evaluated MSI in 97 cases enrolled for endoscopy of upper GI tract with symptoms of dyspepsia, reflux or dysphagia. We aimed at evaluating markers that reflect instability in esophageal malignancies, examine the prevalence of MSI in cancers and other pathologies of the esophagus, and determine the methylation status of hMLH1 gene in relation to MSI. 42% (21/50) cancers and 15.4%(2/13) precancers exhibited MSI where 85.7% cancers and 50% precancers with MSI, showed a hypermethylated hMLH1 promoter.	topic_ccc
74458	6	354914	7	NULL	NULL	NULL	NULL	statement 4	Process		involves					hMLH1	GP	hypermethylated		promoter	NULL		NULL	NULL	NULL	NULL	NULL	NULL	Instability at microsatellite loci is widely attributed to mismatch repair errors due to epigenetic alterations. Using three dinucleotide markers, D3S1313, D9S171, D17S250 and two mononucleotide markers BAT25, BATRII, we evaluated MSI in 97 cases enrolled for endoscopy of upper GI tract with symptoms of dyspepsia, reflux or dysphagia. We aimed at evaluating markers that reflect instability in esophageal malignancies, examine the prevalence of MSI in cancers and other pathologies of the esophagus, and determine the methylation status of hMLH1 gene in relation to MSI. 42% (21/50) cancers and 15.4%(2/13) precancers exhibited MSI where 85.7% cancers and 50% precancers with MSI, showed a hypermethylated hMLH1 promoter.	topic_ccc
74459	1	354916	7	NULL	NULL	0	NULL	hMLH1	GP	methylation of	correlated with		significantly			p53	GP	high level expression of			NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore, methylation of hMLH1 significantly correlated with high level of P53 expression (P = .006) and with overall survival (P = .015) suggesting that silencing of hMLH1 through aberrant promoter methylation could be used as a poor prognosis indicator in breast cancer.	topic_ccc
74460	2	354916	7	NULL	NULL	0	NULL	hMLH1	GP		silenced through							methylation of		aberrant promoter	NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore, methylation of hMLH1 significantly correlated with high level of P53 expression (P = .006) and with overall survival (P = .015) suggesting that silencing of hMLH1 through aberrant promoter methylation could be used as a poor prognosis indicator in breast cancer.	topic_ccc
74461	3	354916	7	NULL	NULL	0	NULL	statement 2	Process		used as					breast cancer	MedicalFinding	poor prognosis indicator in			NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore, methylation of hMLH1 significantly correlated with high level of P53 expression (P = .006) and with overall survival (P = .015) suggesting that silencing of hMLH1 through aberrant promoter methylation could be used as a poor prognosis indicator in breast cancer.	topic_ccc
74462	1	354917	7	NULL	NULL	0	NULL	hMLH1	GP	hypermethylation of 	is found in				promoter	MSI-H gastric carcinomas	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter hypermethylation of hMLH1, E-cadherin, and p16(INK4A) was found in 89%, 78%, and 33% of MSI-H gastric carcinomas and in 16%, 32%, and 11% of MSS carcinomas, respectively (p = 0.01).	topic_ccc
74463	2	354917	7	NULL	NULL	0	NULL	E-cadheriny	GP	hypermethylation of 	is found in				promoter	MSI-H gastric carcinomas	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter hypermethylation of hMLH1, E-cadherin, and p16(INK4A) was found in 89%, 78%, and 33% of MSI-H gastric carcinomas and in 16%, 32%, and 11% of MSS carcinomas, respectively (p = 0.01).	topic_ccc
74464	3	354917	7	NULL	NULL	0	NULL	p16(INK4A)	GP	hypermethylation of 	is found in				promoter	MSI-H gastric carcinomas	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter hypermethylation of hMLH1, E-cadherin, and p16(INK4A) was found in 89%, 78%, and 33% of MSI-H gastric carcinomas and in 16%, 32%, and 11% of MSS carcinomas, respectively (p = 0.01).	topic_ccc
74465	4	354917	7	NULL	NULL	0	NULL	hMLH1	GP	hypermethylation of 	is found in				promoter	MSS carcinomas	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter hypermethylation of hMLH1, E-cadherin, and p16(INK4A) was found in 89%, 78%, and 33% of MSI-H gastric carcinomas and in 16%, 32%, and 11% of MSS carcinomas, respectively (p = 0.01).	topic_ccc
74466	5	354917	7	NULL	NULL	0	NULL	E-cadherin	GP	hypermethylation of 	is found in				promoter	MSS carcinomas	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter hypermethylation of hMLH1, E-cadherin, and p16(INK4A) was found in 89%, 78%, and 33% of MSI-H gastric carcinomas and in 16%, 32%, and 11% of MSS carcinomas, respectively (p = 0.01).	topic_ccc
74467	6	354917	7	NULL	NULL	0	NULL	p16(INK4A)	GP	hypermethylation of 	is found in				promoter	MSS carcinomas	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter hypermethylation of hMLH1, E-cadherin, and p16(INK4A) was found in 89%, 78%, and 33% of MSI-H gastric carcinomas and in 16%, 32%, and 11% of MSS carcinomas, respectively (p = 0.01).	topic_ccc
74468	1	354918	7	NULL	NULL	0	NULL	BRCA1	GP	methylation of	correlated with					disease free survival	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	BRCA1 methylation correlated with age at diagnosis (P = .015) and 5-years disease free survival (P = .016) while hMLH1 methylation was more frequent in larger tumors (P = .002) and in presence of distant metastasis (P = .004).	topic_ccc
74469	2	354918	7	NULL	NULL	0	NULL	hMLH1	GP	methylation of	is more frequent in					larger tumors	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	BRCA1 methylation correlated with age at diagnosis (P = .015) and 5-years disease free survival (P = .016) while hMLH1 methylation was more frequent in larger tumors (P = .002) and in presence of distant metastasis (P = .004).	topic_ccc
74470	3	354918	7	NULL	NULL	0	NULL	hMLH1	GP	methylation of	is more frequent in					distant metastasis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	BRCA1 methylation correlated with age at diagnosis (P = .015) and 5-years disease free survival (P = .016) while hMLH1 methylation was more frequent in larger tumors (P = .002) and in presence of distant metastasis (P = .004).	topic_ccc
74471	1	354919	7	NULL	NULL	0	NULL	CTCF	GP		contributes to					Rb gene	GP	epigenetic regulation of;;human		promoter	NULL	tumoral cell lines	0	NULL	NULL	NULL	NULL	NULL	Here we addressed the contribution of the multifunctional nuclear factor CTCF to the epigenetic regulation of the human retinoblastoma (Rb) gene promoter in different tumoral cell lines.	topic_ccc
74472	2	354919	7	NULL	NULL	0	NULL	CTCF	GP		is a type of					multifunctional nuclear factor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Here we addressed the contribution of the multifunctional nuclear factor CTCF to the epigenetic regulation of the human retinoblastoma (Rb) gene promoter in different tumoral cell lines.	topic_ccc
74473	3	354919	7	NULL	NULL	0	NULL	Rb	GP		is					retinoblastoma 	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Here we addressed the contribution of the multifunctional nuclear factor CTCF to the epigenetic regulation of the human retinoblastoma (Rb) gene promoter in different tumoral cell lines.	topic_ccc
74474	1	354920	7	NULL	NULL	0	NULL	LW6	Chemical		promotes					HIF-1alpha	GP	proteasomal degradation of			NULL	colon cancer cell line	0	NULL	NULL	NULL	NULL	NULL	LW6, a novel HIF-1 inhibitor, promotes proteasomal degradation of HIF-1alpha via upregulation of VHL in a colon cancer cell line.	topic_ccc
74475	2	354920	7	NULL	NULL	0	NULL	statement 1	Process		via					VHL	GP	upregulation of			NULL	colon cancer cell line	0	NULL	NULL	NULL	NULL	NULL	LW6, a novel HIF-1 inhibitor, promotes proteasomal degradation of HIF-1alpha via upregulation of VHL in a colon cancer cell line.	topic_ccc
74476	3	354920	7	NULL	NULL	0	NULL	LW6	Chemical		is a type of					HIF-1 inhibitor	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	LW6, a novel HIF-1 inhibitor, promotes proteasomal degradation of HIF-1alpha via upregulation of VHL in a colon cancer cell line.	topic_ccc
74478	1	354921	7	NULL	NULL	NULL	NULL	p16INK4A	GP	downregulation of	marker to		possible			retinoblastoma	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Downregulation and aberrant promoter methylation of p16INK4A: a possible novel heritable susceptibility marker to retinoblastoma.	topic_ccc
74479	2	354921	7	NULL	NULL	NULL	NULL	p16INK4A	GP	aberrant methylation of	marker to		possible		promoter	retinoblastoma	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Downregulation and aberrant promoter methylation of p16INK4A: a possible novel heritable susceptibility marker to retinoblastoma.	topic_ccc
74480	3	354921	7	NULL	NULL	0	NULL	p16INK4A	GP		is a type of					novel heritable susceptibility marker	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Downregulation and aberrant promoter methylation of p16INK4A: a possible novel heritable susceptibility marker to retinoblastoma.	topic_ccc
74482	1	354922	7	NULL	NULL	0	NULL	hMLH1 	GP		is involved in					DNA repair	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 In the current study, we aimed to assess by MSP, the methylation pattern of two cancer-related genes involved in DNA repair: hMLH1 (mutL homolog 1, colon cancer, nonpolyposis type 2 (E. coli) and BRCA1 (breast cancer 1, early onset) in 78 primary breast cancers from Tunisian patients.	topic_ccc
74484	2	354922	7	NULL	NULL	0	NULL	BRCA1	GP		is involved in					DNA repair	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 In the current study, we aimed to assess by MSP, the methylation pattern of two cancer-related genes involved in DNA repair: hMLH1 (mutL homolog 1, colon cancer, nonpolyposis type 2 (E. coli) and BRCA1 (breast cancer 1, early onset) in 78 primary breast cancers from Tunisian patients.	topic_ccc
74486	3	354922	7	NULL	NULL	0	NULL	 hMLH1	GP		is					mutL homolog 1	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 In the current study, we aimed to assess by MSP, the methylation pattern of two cancer-related genes involved in DNA repair: hMLH1 (mutL homolog 1, colon cancer, nonpolyposis type 2 (E. coli) and BRCA1 (breast cancer 1, early onset) in 78 primary breast cancers from Tunisian patients.	topic_ccc
74487	4	354922	7	NULL	NULL	0	NULL	BRCA1	GP		is					breast cancer 1, early onset	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 In the current study, we aimed to assess by MSP, the methylation pattern of two cancer-related genes involved in DNA repair: hMLH1 (mutL homolog 1, colon cancer, nonpolyposis type 2 (E. coli) and BRCA1 (breast cancer 1, early onset) in 78 primary breast cancers from Tunisian patients.	topic_ccc
74500	1	354924	7	NULL	NULL	0	NULL	aspirin chemoprevention	Chemical		prevent		maybe;;effective 			colorectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have indicated that aspirin chemoprevention may be effective in preventing colorectal cancer within the general population, and aspirin, celecoxib, and calcium may be effective in preventing adenomas within those people who have previously undergone polypectomy.	topic_ccc
74501	2	354924	7	NULL	NULL	NULL	NULL	aspirin	Chemical		prevent		may be;;effective			adenomas	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Studies have indicated that aspirin chemoprevention may be effective in preventing colorectal cancer within the general population, and aspirin, celecoxib, and calcium may be effective in preventing adenomas within those people who have previously undergone polypectomy.	topic_ccc
74502	3	354924	7	NULL	NULL	0	NULL	celecoxib	Chemical		prevent		maybe;;effective			adenomas	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have indicated that aspirin chemoprevention may be effective in preventing colorectal cancer within the general population, and aspirin, celecoxib, and calcium may be effective in preventing adenomas within those people who have previously undergone polypectomy.	topic_ccc
74503	4	354924	7	NULL	NULL	0	NULL	calcium	Chemical		prevent		maybe;;effective			adenomas	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have indicated that aspirin chemoprevention may be effective in preventing colorectal cancer within the general population, and aspirin, celecoxib, and calcium may be effective in preventing adenomas within those people who have previously undergone polypectomy.	topic_ccc
74504	5	354924	7	NULL	NULL	0	NULL	statement 2	Process		occur in					polypectomy people	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have indicated that aspirin chemoprevention may be effective in preventing colorectal cancer within the general population, and aspirin, celecoxib, and calcium may be effective in preventing adenomas within those people who have previously undergone polypectomy.	topic_ccc
74505	6	354924	7	NULL	NULL	0	NULL	statement 3	Process		occur in					polypectomy people	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have indicated that aspirin chemoprevention may be effective in preventing colorectal cancer within the general population, and aspirin, celecoxib, and calcium may be effective in preventing adenomas within those people who have previously undergone polypectomy.	topic_ccc
74506	7	354924	7	NULL	NULL	0	NULL	statement 4	Process		occur in					polypectomy people	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have indicated that aspirin chemoprevention may be effective in preventing colorectal cancer within the general population, and aspirin, celecoxib, and calcium may be effective in preventing adenomas within those people who have previously undergone polypectomy.	topic_ccc
74507	8	354924	7	NULL	NULL	0	NULL	statement 1	Process		occur in					general population	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have indicated that aspirin chemoprevention may be effective in preventing colorectal cancer within the general population, and aspirin, celecoxib, and calcium may be effective in preventing adenomas within those people who have previously undergone polypectomy.	topic_ccc
74549	1	354925	7	NULL	NULL	0	NULL	folate	Chemical	low level of	associated with		may be			CIMP-low/0 colon tumors	MedicalFinding	increased risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	This molecular pathological epidemiology study suggests that low level intake of folate may be associated with an increased risk of CIMP-low/0 colon tumors, but not that of CIMP-high tumors. 	topic_ccc
74550	2	354925	7	NULL	NULL	0	NULL	folate	Chemical	low level of	is not associated with					CIMP-high tumors	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	This molecular pathological epidemiology study suggests that low level intake of folate may be associated with an increased risk of CIMP-low/0 colon tumors, but not that of CIMP-high tumors. 	topic_ccc
74551	1	354926	7	NULL	NULL	0	NULL	 alcohol	Chemical	frequent consumption of	is associated with					distal colon cancer	MedicalFinding	elevated risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	Frequent alcohol consumption and consuming high amounts of alcohol were associated with elevated risk for distal colon cancer in men and higher risk for rectal cancer in women.	topic_ccc
74552	2	354926	7	NULL	NULL	0	NULL	alcohol	Chemical	consuming high amounts of	is associated with					distal colon cancer	MedicalFinding	elevated risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	Frequent alcohol consumption and consuming high amounts of alcohol were associated with elevated risk for distal colon cancer in men and higher risk for rectal cancer in women.	topic_ccc
74553	3	354926	7	NULL	NULL	0	NULL	statement 1	Process		occur in					men	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Frequent alcohol consumption and consuming high amounts of alcohol were associated with elevated risk for distal colon cancer in men and higher risk for rectal cancer in women.	topic_ccc
74554	4	354926	7	NULL	NULL	0	NULL	statement 2	Process		occur in 					men	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Frequent alcohol consumption and consuming high amounts of alcohol were associated with elevated risk for distal colon cancer in men and higher risk for rectal cancer in women.	topic_ccc
74555	5	354926	7	NULL	NULL	0	NULL	alcohol	Chemical	frequent consumption of	is associated with					rectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Frequent alcohol consumption and consuming high amounts of alcohol were associated with elevated risk for distal colon cancer in men and higher risk for rectal cancer in women.	topic_ccc
74556	6	354926	7	NULL	NULL	0	NULL	alcohol	Chemical	consuming high amounts of	is associated with					rectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Frequent alcohol consumption and consuming high amounts of alcohol were associated with elevated risk for distal colon cancer in men and higher risk for rectal cancer in women.	topic_ccc
74557	7	354926	7	NULL	NULL	0	NULL	statement 5	Process		occur in					women	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Frequent alcohol consumption and consuming high amounts of alcohol were associated with elevated risk for distal colon cancer in men and higher risk for rectal cancer in women.	topic_ccc
74558	8	354926	7	NULL	NULL	0	NULL	statement 6	Process		occur in					women	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Frequent alcohol consumption and consuming high amounts of alcohol were associated with elevated risk for distal colon cancer in men and higher risk for rectal cancer in women.	topic_ccc
74569	1	354927	7	NULL	NULL	NULL	NULL	MTHFR 677C/T genotype	Chromosome	distribution of	present in					cancer group	GroupOfPeople				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Distributions of MTHFR 677C/T genotype and allele frequencies in the individuals with and without metabolic syndrome in the cancer group showed no differences.	topic_ccc
74570	2	354927	7	NULL	NULL	NULL	NULL	statement 1	Process		occur with					metabolic syndrome	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Distributions of MTHFR 677C/T genotype and allele frequencies in the individuals with and without metabolic syndrome in the cancer group showed no differences.	topic_ccc
74571	3	354927	7	NULL	NULL	0	NULL	statement 1	Process		occur without					metabolic syndrome	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Distributions of MTHFR 677C/T genotype and allele frequencies in the individuals with and without metabolic syndrome in the cancer group showed no differences.	topic_ccc
74572	4	354927	7	NULL	NULL	NULL	NULL	MTHFR 677C/T genotype	Chromosome	distribution of;;allele frequencies of	present in					cancer group	GroupOfPeople				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Distributions of MTHFR 677C/T genotype and allele frequencies in the individuals with and without metabolic syndrome in the cancer group showed no differences.	topic_ccc
74573	5	354927	7	NULL	NULL	0	NULL	statement 4	Process		occur with					metabolic syndrome	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Distributions of MTHFR 677C/T genotype and allele frequencies in the individuals with and without metabolic syndrome in the cancer group showed no differences.	topic_ccc
74574	6	354927	7	NULL	NULL	0	NULL	statement 4	Process		occur without					metabolic syndrome	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Distributions of MTHFR 677C/T genotype and allele frequencies in the individuals with and without metabolic syndrome in the cancer group showed no differences.	topic_ccc
74575	7	354927	7	NULL	NULL	0	NULL	statement 2	Process		does not differ from					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Distributions of MTHFR 677C/T genotype and allele frequencies in the individuals with and without metabolic syndrome in the cancer group showed no differences.	topic_ccc
74576	8	354927	7	NULL	NULL	0	NULL	statement 5	Process		does not differ from					statement 6	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Distributions of MTHFR 677C/T genotype and allele frequencies in the individuals with and without metabolic syndrome in the cancer group showed no differences.	topic_ccc
74577	1	354928	7	NULL	NULL	0	NULL	IGF	GP		is required for					carcinogenicity	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-like growth factor (IGF)-I receptor (IGF-IR) signaling is required for carcinogenicity and proliferation of gastrointestinal cancers. 	topic_ccc
74578	2	354928	7	NULL	NULL	0	NULL	statement 1	Process		required for					gastrointestinal cancers	MedicalFinding	proliferation of			NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-like growth factor (IGF)-I receptor (IGF-IR) signaling is required for carcinogenicity and proliferation of gastrointestinal cancers. 	topic_ccc
74579	3	354928	7	NULL	NULL	0	NULL	IGF-IR	GP		is required for					carcinogenicity	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-like growth factor (IGF)-I receptor (IGF-IR) signaling is required for carcinogenicity and proliferation of gastrointestinal cancers. 	topic_ccc
74580	4	354928	7	NULL	NULL	0	NULL	statement 3	Process		required for					gastrointestinal cancers	MedicalFinding	proliferation of			NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-like growth factor (IGF)-I receptor (IGF-IR) signaling is required for carcinogenicity and proliferation of gastrointestinal cancers. 	topic_ccc
74582	5	354928	7	NULL	NULL	0	NULL	IGF	GP		is					Insulin-like growth factor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-like growth factor (IGF)-I receptor (IGF-IR) signaling is required for carcinogenicity and proliferation of gastrointestinal cancers. 	topic_ccc
74583	6	354928	7	NULL	NULL	0	NULL	IGF-IR	GP		is					IGF-I receptor 	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-like growth factor (IGF)-I receptor (IGF-IR) signaling is required for carcinogenicity and proliferation of gastrointestinal cancers. 	topic_ccc
74585	1	354929	7	NULL	NULL	0	NULL	Vitamin D	Chemical	intake of	inversely associated with					colorectal cancer	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	Vitamin D intake and blood 25(OH)D levels were inversely associated with the risk of colorectal cancer in this meta-analysis.	topic_ccc
74586	2	354929	7	NULL	NULL	0	NULL	25(OH)D	Chemical		inversely associated with					colorectal cancer	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	Vitamin D intake and blood 25(OH)D levels were inversely associated with the risk of colorectal cancer in this meta-analysis.	topic_ccc
74587	1	354930	7	NULL	NULL	0	NULL	calcium	Chemical		protective against					 colorectal neoplasia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion, a high calcium intake and the use of calcium supplements may be protective against colorectal neoplasia, although a greater sample may be required to observe significant associations in a multivariate model.	topic_ccc
74588	2	354930	7	NULL	NULL	0	NULL	calcium supplement	Chemical		protective against					colorectal neoplasia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion, a high calcium intake and the use of calcium supplements may be protective against colorectal neoplasia, although a greater sample may be required to observe significant associations in a multivariate model.	topic_ccc
74590	1	354931	7	NULL	NULL	0	NULL	combination chemotherapy	MedicalProcedure		applied in					mCRC	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Several randomized trials have indicated that combination chemotherapy applied in metastatic colorectal cancer (mCRC) does not significantly improve overall survival when compared to the sequential use of cytotoxic agents (CAIRO, MRC Focus, FFCD 2000-05).	topic_ccc
74591	2	354931	7	NULL	NULL	0	NULL	statement 1	Process		does not improve		significantly			survival	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Several randomized trials have indicated that combination chemotherapy applied in metastatic colorectal cancer (mCRC) does not significantly improve overall survival when compared to the sequential use of cytotoxic agents (CAIRO, MRC Focus, FFCD 2000-05).	topic_ccc
74592	3	354931	7	NULL	NULL	0	NULL	mCRC	MedicalFinding		is					metastatic colorectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Several randomized trials have indicated that combination chemotherapy applied in metastatic colorectal cancer (mCRC) does not significantly improve overall survival when compared to the sequential use of cytotoxic agents (CAIRO, MRC Focus, FFCD 2000-05).	topic_ccc
74597	1	354933	7	NULL	NULL	0	NULL	RUNX3	GP	methylation of	occur in				promoter	colorectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	RUNX3 promoter methylation in colorectal cancer: its relationship with microsatellite instability and its suitability as a novel serum tumor marker.	topic_ccc
74598	2	354933	7	NULL	NULL	NULL	NULL	RUNX3	GP	methylation of	is in relation with				promoter	microsatellite instability	Chromosome				NULL		NULL	NULL	NULL	NULL	NULL	NULL	RUNX3 promoter methylation in colorectal cancer: its relationship with microsatellite instability and its suitability as a novel serum tumor marker.	topic_ccc
74599	3	354933	7	NULL	NULL	0	NULL	RUNX3	GP	methylation of	acts as a				promoter	novel serum tumor marker	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	RUNX3 promoter methylation in colorectal cancer: its relationship with microsatellite instability and its suitability as a novel serum tumor marker.	topic_ccc
74600	1	354934	7	NULL	NULL	0	NULL	Epigenetic Gene	GP	methylation of	is associated with				promoter	Child's Later Adiposity	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	 Epigenetic Gene Promoter Methylation at Birth Is Associated With Child's Later Adiposity.	topic_ccc
74601	1	354935	7	NULL	NULL	0	NULL	adenosine A2A receptor	GP	genetic inactivation of	attenuates					pathologic angiogenesis	Process				NULL	mouse retina	0	NULL	NULL	NULL	NULL	NULL	Genetic inactivation of the adenosine A2A receptor attenuates pathologic but not developmental angiogenesis in the mouse retina.	topic_ccc
74602	2	354935	7	NULL	NULL	0	NULL	adenosine A2A receptor	GP	genetic inactivation of	does not attenuate					developmental angiogenesis	Process				NULL	mouse retina	0	NULL	NULL	NULL	NULL	NULL	Genetic inactivation of the adenosine A2A receptor attenuates pathologic but not developmental angiogenesis in the mouse retina.	topic_ccc
74603	1	354936	7	NULL	NULL	NULL	NULL	 MTHFR C677T 	Chemical	Functional polymorphisms of	affect					toxicity	Process	outcome of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional polymorphisms of MTHFR C677T and MTR A2756G can affect outcome and risk of toxicity during adjuvant chemotherapy in stage III colorectal cancer.	topic_ccc
74604	2	354936	7	NULL	NULL	0	NULL	MTR A2756G	Chemical	Functional polymorphisms of	affect					toxicity	Process	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	Functional polymorphisms of MTHFR C677T and MTR A2756G can affect outcome and risk of toxicity during adjuvant chemotherapy in stage III colorectal cancer.	topic_ccc
74605	3	354936	7	NULL	NULL	0	NULL	statement 1	Process		occur during					stage III colorectal cancer	MedicalFinding	adjuvant chemotherapy in			NULL		0	NULL	NULL	NULL	NULL	NULL	Functional polymorphisms of MTHFR C677T and MTR A2756G can affect outcome and risk of toxicity during adjuvant chemotherapy in stage III colorectal cancer.	topic_ccc
74606	4	354936	7	NULL	NULL	0	NULL	statement 2	Process		occur during					stage III colorectal cancer	MedicalFinding	adjuvant chemotherapy in			NULL		0	NULL	NULL	NULL	NULL	NULL	Functional polymorphisms of MTHFR C677T and MTR A2756G can affect outcome and risk of toxicity during adjuvant chemotherapy in stage III colorectal cancer.	topic_ccc
74721	1	354937	7	NULL	NULL	0	NULL	MDR1 gene	GP		transcriptional target of 		direct			CDX2	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence that the MDR1 gene was a direct transcriptional target of CDX2 was obtained, including analyses with MDR1 reporter gene constructs and chromatin immunoprecipitation assays.	topic_ccc
74722	1	354938	7	NULL	NULL	0	NULL	Bcl-2	GP		hypomethlated in				promoter	colorectal cancer tissue	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Bcl-2 promoter is hypomethylated in colorectal cancer tissue, and there is a significant correlation between MTHFR 677 TT or CT/TT genotypes and CRC or Bcl-2 promoter CGI methylation/oncoprotein expression in CRC.	topic_ccc
74723	2	354938	7	NULL	NULL	NULL	NULL	MTHFR 677 TT genotype	PhysicalPhenomenon		correlates with		significantly			CRC 	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bcl-2 promoter is hypomethylated in colorectal cancer tissue, and there is a significant correlation between MTHFR 677 TT or CT/TT genotypes and CRC or Bcl-2 promoter CGI methylation/oncoprotein expression in CRC.	topic_ccc
74724	3	354938	7	NULL	NULL	NULL	NULL	CT/TT genotype	PhysicalPhenomenon		correlates with		significantly			CRC	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bcl-2 promoter is hypomethylated in colorectal cancer tissue, and there is a significant correlation between MTHFR 677 TT or CT/TT genotypes and CRC or Bcl-2 promoter CGI methylation/oncoprotein expression in CRC.	topic_ccc
74725	4	354938	7	NULL	NULL	NULL	NULL	MTHFR 677 TT genotype	PhysicalPhenomenon		correlates with		significantly			Bcl-2	GP			promoter CGI methylation	NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bcl-2 promoter is hypomethylated in colorectal cancer tissue, and there is a significant correlation between MTHFR 677 TT or CT/TT genotypes and CRC or Bcl-2 promoter CGI methylation/oncoprotein expression in CRC.	topic_ccc
74726	5	354938	7	NULL	NULL	NULL	NULL	CT/TT genotype	PhysicalPhenomenon		correlates with		significantly			Bcl2	GP			promoter CGI methylation	NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bcl-2 promoter is hypomethylated in colorectal cancer tissue, and there is a significant correlation between MTHFR 677 TT or CT/TT genotypes and CRC or Bcl-2 promoter CGI methylation/oncoprotein expression in CRC.	topic_ccc
74727	6	354938	7	NULL	NULL	0	NULL	statement 4	Process		occur in					CRC	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Bcl-2 promoter is hypomethylated in colorectal cancer tissue, and there is a significant correlation between MTHFR 677 TT or CT/TT genotypes and CRC or Bcl-2 promoter CGI methylation/oncoprotein expression in CRC.	topic_ccc
74728	7	354938	7	NULL	NULL	0	NULL	statement 5	Process		occur in					CRC	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Bcl-2 promoter is hypomethylated in colorectal cancer tissue, and there is a significant correlation between MTHFR 677 TT or CT/TT genotypes and CRC or Bcl-2 promoter CGI methylation/oncoprotein expression in CRC.	topic_ccc
74729	8	354938	7	NULL	NULL	0	NULL	MTHFR 677 TT genotype	PhysicalPhenomenon		correlates with		significantly			Bcl-2	GP	oncoprotein expression		promoter 	NULL		0	NULL	NULL	NULL	NULL	NULL	Bcl-2 promoter is hypomethylated in colorectal cancer tissue, and there is a significant correlation between MTHFR 677 TT or CT/TT genotypes and CRC or Bcl-2 promoter CGI methylation/oncoprotein expression in CRC.	topic_ccc
74730	9	354938	7	NULL	NULL	0	NULL	CT/TT genotype	PhysicalPhenomenon		correlates with		significantly			Bcl-2	GP	oncoprotein expression		promoter	NULL		0	NULL	NULL	NULL	NULL	NULL	Bcl-2 promoter is hypomethylated in colorectal cancer tissue, and there is a significant correlation between MTHFR 677 TT or CT/TT genotypes and CRC or Bcl-2 promoter CGI methylation/oncoprotein expression in CRC.	topic_ccc
74731	10	354938	7	NULL	NULL	0	NULL	statement 8	Process		occur in					CRC	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Bcl-2 promoter is hypomethylated in colorectal cancer tissue, and there is a significant correlation between MTHFR 677 TT or CT/TT genotypes and CRC or Bcl-2 promoter CGI methylation/oncoprotein expression in CRC.	topic_ccc
74732	11	354938	7	NULL	NULL	0	NULL	statement 9	Process		occur in					CRC 	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Bcl-2 promoter is hypomethylated in colorectal cancer tissue, and there is a significant correlation between MTHFR 677 TT or CT/TT genotypes and CRC or Bcl-2 promoter CGI methylation/oncoprotein expression in CRC.	topic_ccc
74733	1	354939	7	NULL	NULL	0	NULL	Fluoropyrimidine-based combination chemotherapy	MedicalProcedure		has efficacy in					ACC	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	Fluoropyrimidine-based combination chemotherapy, in combination with either oxaliplatin or irinotecan, has demonstrated efficacy and tolerability in treatment of advanced colorectal cancer (ACC).	topic_ccc
74734	2	354939	7	NULL	NULL	NULL	NULL	Fluoropyrimidine-based combination chemotherapy	MedicalProcedure		has  tolerability in					ACC	MedicalFinding	treatment of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fluoropyrimidine-based combination chemotherapy, in combination with either oxaliplatin or irinotecan, has demonstrated efficacy and tolerability in treatment of advanced colorectal cancer (ACC).	topic_ccc
74735	3	354939	7	NULL	NULL	0	NULL	ACC	MedicalFinding		is					advanced colorectal cancer 	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Fluoropyrimidine-based combination chemotherapy, in combination with either oxaliplatin or irinotecan, has demonstrated efficacy and tolerability in treatment of advanced colorectal cancer (ACC).	topic_ccc
74736	4	354939	7	NULL	NULL	0	NULL	statement 1	Process		in combination with					oxaliplatin 	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Fluoropyrimidine-based combination chemotherapy, in combination with either oxaliplatin or irinotecan, has demonstrated efficacy and tolerability in treatment of advanced colorectal cancer (ACC).	topic_ccc
74737	5	354939	7	NULL	NULL	NULL	NULL	statement 1	Process		in combination with					irinotecan	Chemical				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fluoropyrimidine-based combination chemotherapy, in combination with either oxaliplatin or irinotecan, has demonstrated efficacy and tolerability in treatment of advanced colorectal cancer (ACC).	topic_ccc
74738	6	354939	7	NULL	NULL	0	NULL	statement 2	Process		in combination with					oxaliplatin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Fluoropyrimidine-based combination chemotherapy, in combination with either oxaliplatin or irinotecan, has demonstrated efficacy and tolerability in treatment of advanced colorectal cancer (ACC).	topic_ccc
74739	7	354939	7	NULL	NULL	0	NULL	statement 2	Process		in combination with					 irinotecan	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Fluoropyrimidine-based combination chemotherapy, in combination with either oxaliplatin or irinotecan, has demonstrated efficacy and tolerability in treatment of advanced colorectal cancer (ACC).	topic_ccc
74740	1	354940	7	NULL	NULL	NULL	NULL	APC	GP	epigenetic gene silencing of	play a role in					CRC	MedicalFinding	development of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	We examined the paired tumour and normal-tissue specimens of 86 CRC patients for the occurrence of aberrations in the mutation cluster region (MCR) of the APC gene and exon 3 of the β-catenin gene by polymerase chain reaction-single-strand conformation polymorphism (PCR-SSCP) and/or PCR-direct sequencing. Although the number of mutations in the APC and β-catenin genes in our CRC cases was very low, the study confirms the role of epigenetic gene silencing of the pivotal molecular gladiator, APC, of the Wnt pathway in the development of CRC in the Kashmiri population.	topic_ccc
74741	2	354940	7	NULL	NULL	0	NULL	APC	GP		is a type of					pivotal molecular gladiator	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	We examined the paired tumour and normal-tissue specimens of 86 CRC patients for the occurrence of aberrations in the mutation cluster region (MCR) of the APC gene and exon 3 of the β-catenin gene by polymerase chain reaction-single-strand conformation polymorphism (PCR-SSCP) and/or PCR-direct sequencing. Although the number of mutations in the APC and β-catenin genes in our CRC cases was very low, the study confirms the role of epigenetic gene silencing of the pivotal molecular gladiator, APC, of the Wnt pathway in the development of CRC in the Kashmiri population.	topic_ccc
74742	3	354940	7	NULL	NULL	0	NULL	APC	GP		belongs to					Wnt pathway	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	We examined the paired tumour and normal-tissue specimens of 86 CRC patients for the occurrence of aberrations in the mutation cluster region (MCR) of the APC gene and exon 3 of the β-catenin gene by polymerase chain reaction-single-strand conformation polymorphism (PCR-SSCP) and/or PCR-direct sequencing. Although the number of mutations in the APC and β-catenin genes in our CRC cases was very low, the study confirms the role of epigenetic gene silencing of the pivotal molecular gladiator, APC, of the Wnt pathway in the development of CRC in the Kashmiri population.	topic_ccc
74743	4	354940	7	NULL	NULL	0	NULL	statement 1	Process		occur in					Kashmiri population	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	We examined the paired tumour and normal-tissue specimens of 86 CRC patients for the occurrence of aberrations in the mutation cluster region (MCR) of the APC gene and exon 3 of the β-catenin gene by polymerase chain reaction-single-strand conformation polymorphism (PCR-SSCP) and/or PCR-direct sequencing. Although the number of mutations in the APC and β-catenin genes in our CRC cases was very low, the study confirms the role of epigenetic gene silencing of the pivotal molecular gladiator, APC, of the Wnt pathway in the development of CRC in the Kashmiri population.	topic_ccc
74744	1	354941	7	NULL	NULL	0	NULL	COX-1	GP		expressed in		constitutively 			normal tissue	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	COX-1 is constitutively expressed in normal tissue, serving an important role in tissue homeostasis, whereas COX-2 is an inducible enzyme, which is markedly overexpressed at sites of inflammation and colorectal neoplasms\t	topic_ccc
74745	2	354941	7	NULL	NULL	0	NULL	statement 1	Process		important role in					tissue homeostasis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	COX-1 is constitutively expressed in normal tissue, serving an important role in tissue homeostasis, whereas COX-2 is an inducible enzyme, which is markedly overexpressed at sites of inflammation and colorectal neoplasms\t	topic_ccc
74746	3	354941	7	NULL	NULL	0	NULL	 COX-2 	GP		is a type of					inducible enzyme	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	COX-1 is constitutively expressed in normal tissue, serving an important role in tissue homeostasis, whereas COX-2 is an inducible enzyme, which is markedly overexpressed at sites of inflammation and colorectal neoplasms\t	topic_ccc
74747	4	354941	7	NULL	NULL	0	NULL	COX-2	GP		overexpressed at		markedly			sites of inflammation	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	COX-1 is constitutively expressed in normal tissue, serving an important role in tissue homeostasis, whereas COX-2 is an inducible enzyme, which is markedly overexpressed at sites of inflammation and colorectal neoplasms\t	topic_ccc
74748	5	354941	7	NULL	NULL	0	NULL	COX-2	GP		overexpressed at		markedly			colorectal neoplasms	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	COX-1 is constitutively expressed in normal tissue, serving an important role in tissue homeostasis, whereas COX-2 is an inducible enzyme, which is markedly overexpressed at sites of inflammation and colorectal neoplasms\t	topic_ccc
74749	1	354942	7	NULL	NULL	0	NULL	sulindac 	Chemical		exert their		may			anti-neoplastic role	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	It may be stated that sulindac and celecoxib, the two NSAIDs may exert their anti-neoplastic role in colorectal cancer via modifying the physicochemical properties of the membranes. http://www.ncbi.nlm.nih.gov/pubmed/21725642	topic_ccc
74750	2	354942	7	NULL	NULL	0	NULL	celecoxib	Chemical		exert their		may			anti-neoplastic role	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	It may be stated that sulindac and celecoxib, the two NSAIDs may exert their anti-neoplastic role in colorectal cancer via modifying the physicochemical properties of the membranes. http://www.ncbi.nlm.nih.gov/pubmed/21725642	topic_ccc
74751	3	354942	7	NULL	NULL	0	NULL	statement 1	Process		occur in					colorectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	It may be stated that sulindac and celecoxib, the two NSAIDs may exert their anti-neoplastic role in colorectal cancer via modifying the physicochemical properties of the membranes. http://www.ncbi.nlm.nih.gov/pubmed/21725642	topic_ccc
74752	4	354942	7	NULL	NULL	0	NULL	statement 2	Process		occur in					colorectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	It may be stated that sulindac and celecoxib, the two NSAIDs may exert their anti-neoplastic role in colorectal cancer via modifying the physicochemical properties of the membranes. http://www.ncbi.nlm.nih.gov/pubmed/21725642	topic_ccc
74753	5	354942	7	NULL	NULL	0	NULL	statement 1	Process		occur via					membrane	CellComponent	modifying the physicochemical properties of			NULL		0	NULL	NULL	NULL	NULL	NULL	It may be stated that sulindac and celecoxib, the two NSAIDs may exert their anti-neoplastic role in colorectal cancer via modifying the physicochemical properties of the membranes. http://www.ncbi.nlm.nih.gov/pubmed/21725642	topic_ccc
74754	6	354942	7	NULL	NULL	0	NULL	statement 2	Process		occur via					membrane	CellComponent	modifying the physicochemical properties of 			NULL		0	NULL	NULL	NULL	NULL	NULL	It may be stated that sulindac and celecoxib, the two NSAIDs may exert their anti-neoplastic role in colorectal cancer via modifying the physicochemical properties of the membranes. http://www.ncbi.nlm.nih.gov/pubmed/21725642	topic_ccc
74755	7	354942	7	NULL	NULL	0	NULL	sulindac	Chemical		is a type of					NSAID	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	It may be stated that sulindac and celecoxib, the two NSAIDs may exert their anti-neoplastic role in colorectal cancer via modifying the physicochemical properties of the membranes. http://www.ncbi.nlm.nih.gov/pubmed/21725642	topic_ccc
74756	8	354942	7	NULL	NULL	0	NULL	celecoxib	Chemical		is a type of					NSAID	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	It may be stated that sulindac and celecoxib, the two NSAIDs may exert their anti-neoplastic role in colorectal cancer via modifying the physicochemical properties of the membranes. http://www.ncbi.nlm.nih.gov/pubmed/21725642	topic_ccc
74757	1	354943	7	NULL	NULL	0	NULL	Energy consumption	Process		influence					colorectal cancer	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	Energy consumption also influences colorectal cancer risk, with obesity increasing risk and exercise reducing risk. 	topic_ccc
74758	2	354943	7	NULL	NULL	0	NULL	Energy consumption	Process		influence					obesity	MedicalFinding	increasing risk of 			NULL		0	NULL	NULL	NULL	NULL	NULL	Energy consumption also influences colorectal cancer risk, with obesity increasing risk and exercise reducing risk. 	topic_ccc
74759	3	354943	7	NULL	NULL	0	NULL	Energy consumption	Process		influence					exercise	Process	reducing risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	Energy consumption also influences colorectal cancer risk, with obesity increasing risk and exercise reducing risk. 	topic_ccc
74760	1	354944	7	NULL	NULL	0	NULL	S100A4 	GP		target gene of					Wnt/β-catenin pathway	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	S100A4 is a target gene of the Wnt/β-catenin pathway, which is constitutively active in the majority of colon cancers.	topic_ccc
74761	2	354944	7	NULL	NULL	0	NULL	statement 1	Process		active in		constitutively 			colon cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	S100A4 is a target gene of the Wnt/β-catenin pathway, which is constitutively active in the majority of colon cancers.	topic_ccc
74762	1	354945	7	NULL	NULL	0	NULL	Obesity	MedicalFinding		influence					colorectal cancer	MedicalFinding	risk of developing			NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity, consumption of red meat, a Western pattern diet, alcohol, and smoking influence one's risk of developing colorectal cancer while physical activity, vitamin D, postmenopausal estrogen use, aspirin, and nonsteroidal anti-inflammatory drugs (NSAIDs) decrease one's risk. 	topic_ccc
74763	2	354945	7	NULL	NULL	0	NULL	red meat	Food		influence					colorectal cancer	MedicalFinding	risk of developing			NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity, consumption of red meat, a Western pattern diet, alcohol, and smoking influence one's risk of developing colorectal cancer while physical activity, vitamin D, postmenopausal estrogen use, aspirin, and nonsteroidal anti-inflammatory drugs (NSAIDs) decrease one's risk. 	topic_ccc
74764	3	354945	7	NULL	NULL	0	NULL	Western pattern diet	Food		influence					colorectal cancer	MedicalFinding	risk of developing			NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity, consumption of red meat, a Western pattern diet, alcohol, and smoking influence one's risk of developing colorectal cancer while physical activity, vitamin D, postmenopausal estrogen use, aspirin, and nonsteroidal anti-inflammatory drugs (NSAIDs) decrease one's risk. 	topic_ccc
74765	4	354945	7	NULL	NULL	0	NULL	alcohol	Chemical		influence					colorectal cancer	MedicalFinding	risk of developing			NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity, consumption of red meat, a Western pattern diet, alcohol, and smoking influence one's risk of developing colorectal cancer while physical activity, vitamin D, postmenopausal estrogen use, aspirin, and nonsteroidal anti-inflammatory drugs (NSAIDs) decrease one's risk. 	topic_ccc
74766	5	354945	7	NULL	NULL	0	NULL	smoking	Chemical		influence					colorectal cancer	MedicalFinding	risk of developing			NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity, consumption of red meat, a Western pattern diet, alcohol, and smoking influence one's risk of developing colorectal cancer while physical activity, vitamin D, postmenopausal estrogen use, aspirin, and nonsteroidal anti-inflammatory drugs (NSAIDs) decrease one's risk. 	topic_ccc
74767	6	354945	7	NULL	NULL	0	NULL	physical activity	Process		decrease					colorectal cancer	MedicalFinding	risk of developing			NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity, consumption of red meat, a Western pattern diet, alcohol, and smoking influence one's risk of developing colorectal cancer while physical activity, vitamin D, postmenopausal estrogen use, aspirin, and nonsteroidal anti-inflammatory drugs (NSAIDs) decrease one's risk. 	topic_ccc
74768	7	354945	7	NULL	NULL	0	NULL	Vitamin D	Chemical		decrease					colorectal cancer	MedicalFinding	risk of developing			NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity, consumption of red meat, a Western pattern diet, alcohol, and smoking influence one's risk of developing colorectal cancer while physical activity, vitamin D, postmenopausal estrogen use, aspirin, and nonsteroidal anti-inflammatory drugs (NSAIDs) decrease one's risk. 	topic_ccc
74769	8	354945	7	NULL	NULL	0	NULL	postmenopausal estrogen use	Chemical		decrease					colorectal cancer	MedicalFinding	risk of developing			NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity, consumption of red meat, a Western pattern diet, alcohol, and smoking influence one's risk of developing colorectal cancer while physical activity, vitamin D, postmenopausal estrogen use, aspirin, and nonsteroidal anti-inflammatory drugs (NSAIDs) decrease one's risk. 	topic_ccc
74770	9	354945	7	NULL	NULL	0	NULL	aspirin	Chemical		decrease					colorectal cancer	MedicalFinding	risk of developing			NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity, consumption of red meat, a Western pattern diet, alcohol, and smoking influence one's risk of developing colorectal cancer while physical activity, vitamin D, postmenopausal estrogen use, aspirin, and nonsteroidal anti-inflammatory drugs (NSAIDs) decrease one's risk. 	topic_ccc
74771	10	354945	7	NULL	NULL	0	NULL	NSAIDs	Chemical		decrease					colorectal cancer	MedicalFinding	risk of developing			NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity, consumption of red meat, a Western pattern diet, alcohol, and smoking influence one's risk of developing colorectal cancer while physical activity, vitamin D, postmenopausal estrogen use, aspirin, and nonsteroidal anti-inflammatory drugs (NSAIDs) decrease one's risk. 	topic_ccc
74772	11	354945	7	NULL	NULL	0	NULL	NSAIDs	Chemical		is					nonsteroidal anti-inflammatory drugs	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity, consumption of red meat, a Western pattern diet, alcohol, and smoking influence one's risk of developing colorectal cancer while physical activity, vitamin D, postmenopausal estrogen use, aspirin, and nonsteroidal anti-inflammatory drugs (NSAIDs) decrease one's risk. 	topic_ccc
74773	1	354946	7	NULL	NULL	0	NULL	colorectal cancer patients 	GroupOfPeople		benefit from					bevacizumab therapy	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	vascular endothelial growth factor-A, thymidylate synthase, and tissue inhibitor of metalloproteinase 3 may enable selection of colorectal cancer patients who would benefit from bevacizumab therapy.	topic_ccc
74774	2	354946	7	NULL	NULL	0	NULL	vascular endothelial growth factor-A	GP		enable		may			statement 1	Process	selection of			NULL		0	NULL	NULL	NULL	NULL	NULL	vascular endothelial growth factor-A, thymidylate synthase, and tissue inhibitor of metalloproteinase 3 may enable selection of colorectal cancer patients who would benefit from bevacizumab therapy.	topic_ccc
74775	3	354946	7	NULL	NULL	0	NULL	thymidylate synthase	GP		enable		may			statement 1	Process	selection of			NULL		0	NULL	NULL	NULL	NULL	NULL	vascular endothelial growth factor-A, thymidylate synthase, and tissue inhibitor of metalloproteinase 3 may enable selection of colorectal cancer patients who would benefit from bevacizumab therapy.	topic_ccc
74776	4	354946	7	NULL	NULL	NULL	NULL	tissue inhibitor of metalloproteinase 3	GP		enable		may			statement 1	Process	selection of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	vascular endothelial growth factor-A, thymidylate synthase, and tissue inhibitor of metalloproteinase 3 may enable selection of colorectal cancer patients who would benefit from bevacizumab therapy.	topic_ccc
74777	1	354947	7	NULL	NULL	NULL	NULL	Microsatellite instability 	NucleicAcid		important factor 					patient survival	Process	associated with			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Microsatellite instability is an important factor associated with patient survival in Chinese sporadic colorectal cancer.	topic_ccc
74790	2	354947	7	NULL	NULL	0	NULL	statement 1	Process		occur in					Chinese sporadic colorectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Microsatellite instability is an important factor associated with patient survival in Chinese sporadic colorectal cancer.	topic_ccc
74793	1	354948	7	NULL	NULL	0	NULL	MGMT	GP	aberrant methylation of	correlates with					MGMT	GP	loss of expression of			NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical analysis revealed abnormal hMLH1 (14, 12.5%), hMSH2 (11, 9.8%), and MGMT (53, 47.3%) expression with a significant correlation between aberrant MGMT methylation and a loss of MGMT expression.	topic_ccc
74794	2	354948	7	NULL	NULL	0	NULL	hMLH1	GP	abnormal expression of	correlates with		significantly			statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical analysis revealed abnormal hMLH1 (14, 12.5%), hMSH2 (11, 9.8%), and MGMT (53, 47.3%) expression with a significant correlation between aberrant MGMT methylation and a loss of MGMT expression.	topic_ccc
74795	3	354948	7	NULL	NULL	NULL	NULL	hMSH2	GP	abnormal expression of	correlates with		significantly			statement 1	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunohistochemical analysis revealed abnormal hMLH1 (14, 12.5%), hMSH2 (11, 9.8%), and MGMT (53, 47.3%) expression with a significant correlation between aberrant MGMT methylation and a loss of MGMT expression.	topic_ccc
74796	4	354948	7	NULL	NULL	0	NULL	MGMT	GP	abnormal expression of	correlates with		significantly			statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical analysis revealed abnormal hMLH1 (14, 12.5%), hMSH2 (11, 9.8%), and MGMT (53, 47.3%) expression with a significant correlation between aberrant MGMT methylation and a loss of MGMT expression.	topic_ccc
74797	1	354949	7	NULL	NULL	NULL	NULL	CIMP	PhysicalPhenomenon		characterized by					p16	GP	abnormal methylation of		multiple CpG islands	NULL		NULL	NULL	NULL	NULL	NULL	NULL	CpG island methylator phenotype (CIMP) in colorectal cancers is characterized by abnormal methylation of multiple CpG islands including those in several tumor suppressor genes such as p16, hMLH1, and THBS1. 	topic_ccc
74798	4	354949	7	NULL	NULL	NULL	NULL	statement 1	Process		occur in					colorectal cancer	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	CpG island methylator phenotype (CIMP) in colorectal cancers is characterized by abnormal methylation of multiple CpG islands including those in several tumor suppressor genes such as p16, hMLH1, and THBS1. 	topic_ccc
74799	2	354949	7	NULL	NULL	NULL	NULL	CIMP	PhysicalPhenomenon		characterized by					hMLH1	GP	abnormal methylation of		multiple CpG islands	NULL		NULL	NULL	NULL	NULL	NULL	NULL	CpG island methylator phenotype (CIMP) in colorectal cancers is characterized by abnormal methylation of multiple CpG islands including those in several tumor suppressor genes such as p16, hMLH1, and THBS1. 	topic_ccc
74800	3	354949	7	NULL	NULL	0	NULL	CIMP	PhysicalPhenomenon		characterized by					THBS1	GP	abnormal methylation of		multiple CpG islands	NULL		0	NULL	NULL	NULL	NULL	NULL	CpG island methylator phenotype (CIMP) in colorectal cancers is characterized by abnormal methylation of multiple CpG islands including those in several tumor suppressor genes such as p16, hMLH1, and THBS1. 	topic_ccc
74801	5	354949	7	NULL	NULL	0	NULL	statement 2	Process		occur in					colorectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	CpG island methylator phenotype (CIMP) in colorectal cancers is characterized by abnormal methylation of multiple CpG islands including those in several tumor suppressor genes such as p16, hMLH1, and THBS1. 	topic_ccc
74802	6	354949	7	NULL	NULL	0	NULL	statement 3	Process		occur in					colorectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	CpG island methylator phenotype (CIMP) in colorectal cancers is characterized by abnormal methylation of multiple CpG islands including those in several tumor suppressor genes such as p16, hMLH1, and THBS1. 	topic_ccc
74803	7	354949	7	NULL	NULL	0	NULL	CIMP	PhysicalPhenomenon		is					CpG island methylator phenotype	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	NULL	NULL	CpG island methylator phenotype (CIMP) in colorectal cancers is characterized by abnormal methylation of multiple CpG islands including those in several tumor suppressor genes such as p16, hMLH1, and THBS1. 	topic_ccc
74804	8	354949	7	NULL	NULL	0	NULL	p16	GP		is a type of					tumor suppressor gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	CpG island methylator phenotype (CIMP) in colorectal cancers is characterized by abnormal methylation of multiple CpG islands including those in several tumor suppressor genes such as p16, hMLH1, and THBS1. 	topic_ccc
74805	9	354949	7	NULL	NULL	0	NULL	hMLH1	GP		is a type of					tumor suppressor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	CpG island methylator phenotype (CIMP) in colorectal cancers is characterized by abnormal methylation of multiple CpG islands including those in several tumor suppressor genes such as p16, hMLH1, and THBS1. 	topic_ccc
74806	10	354949	7	NULL	NULL	0	NULL	THBS1	GP		is a type of					tumor suppressor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	CpG island methylator phenotype (CIMP) in colorectal cancers is characterized by abnormal methylation of multiple CpG islands including those in several tumor suppressor genes such as p16, hMLH1, and THBS1. 	topic_ccc
74807	1	354950	7	NULL	NULL	0	NULL	THBSI	GP		methylated in		frequently			adenomas	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	 THBSI was the most frequently methylated locus in both adenomas (n = 19, 47.5%) and carcinomas (n = 16, 44.4%).	topic_ccc
74808	1	354951	7	NULL	NULL	NULL	NULL	FAK activity	Process	induction of	occur					Wnt	GP	downstream of			NULL	mouse intestine	NULL	NULL	NULL	NULL	NULL	NULL	In contrast, in the mouse intestine, FAK activity was induced downstream of Wnt to promote intestinal regeneration and was also essential for tumorigenesis in an APC deletion model of colorectal cancer. Adding to this complexity, in human cell lines, FAK induced a context-dependent modulation of Wnt signaling to activate target-gene expression.	topic_ccc
74809	2	354951	7	NULL	NULL	NULL	NULL	statement 1	Process		promote					intestinal regeneration	Process				NULL	mouse intestine	NULL	NULL	NULL	NULL	NULL	NULL	In contrast, in the mouse intestine, FAK activity was induced downstream of Wnt to promote intestinal regeneration and was also essential for tumorigenesis in an APC deletion model of colorectal cancer. Adding to this complexity, in human cell lines, FAK induced a context-dependent modulation of Wnt signaling to activate target-gene expression.	topic_ccc
74810	3	354951	7	NULL	NULL	0	NULL	statement 1	Process		essential for					tumorigenesis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast, in the mouse intestine, FAK activity was induced downstream of Wnt to promote intestinal regeneration and was also essential for tumorigenesis in an APC deletion model of colorectal cancer. Adding to this complexity, in human cell lines, FAK induced a context-dependent modulation of Wnt signaling to activate target-gene expression.	topic_ccc
74811	4	354951	7	NULL	NULL	0	NULL	statement 1	Process		occur in					colorectal cancer	MedicalFinding	APC deletion model of 			NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast, in the mouse intestine, FAK activity was induced downstream of Wnt to promote intestinal regeneration and was also essential for tumorigenesis in an APC deletion model of colorectal cancer. Adding to this complexity, in human cell lines, FAK induced a context-dependent modulation of Wnt signaling to activate target-gene expression.	topic_ccc
74812	5	354951	7	NULL	NULL	0	NULL	FAK	GP		induce					Wnt signaling	Process	context-dependent modulation of			NULL	human cell lines	0	NULL	NULL	NULL	NULL	NULL	In contrast, in the mouse intestine, FAK activity was induced downstream of Wnt to promote intestinal regeneration and was also essential for tumorigenesis in an APC deletion model of colorectal cancer. Adding to this complexity, in human cell lines, FAK induced a context-dependent modulation of Wnt signaling to activate target-gene expression.	topic_ccc
74813	6	354951	7	NULL	NULL	0	NULL	statement 5	Process		activate					target-gene 	GP	expression of			NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast, in the mouse intestine, FAK activity was induced downstream of Wnt to promote intestinal regeneration and was also essential for tumorigenesis in an APC deletion model of colorectal cancer. Adding to this complexity, in human cell lines, FAK induced a context-dependent modulation of Wnt signaling to activate target-gene expression.	topic_ccc
74814	1	354952	7	NULL	NULL	0	NULL	PGE2	GP		activate					p38MAPK	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 In addition, PGE2 is able to activate p38 MAPK and the inhibition of p38 MAPK	topic_ccc
74815	1	354953	7	NULL	NULL	0	NULL	17beta-estradiol	Chemical		inhibit					PGE2	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	However, it is unknown if 17beta-estradiol treatment is sufficient to inhibit prostaglandin E2 (PGE2)	topic_ccc
74816	2	354953	7	NULL	NULL	0	NULL	PGE2	Chemical		is					prostaglandin E2	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	However, it is unknown if 17beta-estradiol treatment is sufficient to inhibit prostaglandin E2 (PGE2)	topic_ccc
74817	1	354954	7	NULL	NULL	0	NULL	MapK	GP	activation of	occur in					large intestinal adenomas	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The large intestinal adenomas showed immunohistochemical evidence of activation of MapK	topic_ccc
74818	1	354955	7	NULL	NULL	0	NULL	 SDF-1	GP		induce					uPA	GP	expression of			NULL		0	NULL	NULL	NULL	NULL	NULL	xperiments involving specific inhibitors and small interfering RNA demonstrated that the activation of p38 mitogen-activated protein kinase (MAPK) and phosphatidylinositol 3-kinase (PI3K)/Akt pathways are critical for SDF-1-induced uPA expression.	topic_ccc
74819	2	354955	7	NULL	NULL	0	NULL	p38 mitogen-activated protein kinase	GP	activation of	critical for					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	xperiments involving specific inhibitors and small interfering RNA demonstrated that the activation of p38 mitogen-activated protein kinase (MAPK) and phosphatidylinositol 3-kinase (PI3K)/Akt pathways are critical for SDF-1-induced uPA expression.	topic_ccc
74825	3	354955	7	NULL	NULL	0	NULL	PI3K/Akt pathways	Process	activation of	critical for					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	xperiments involving specific inhibitors and small interfering RNA demonstrated that the activation of p38 mitogen-activated protein kinase (MAPK) and phosphatidylinositol 3-kinase (PI3K)/Akt pathways are critical for SDF-1-induced uPA expression.	topic_ccc
74826	4	354955	7	NULL	NULL	0	NULL	MAPK	GP		is					mitogen-activated protein kinase	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	xperiments involving specific inhibitors and small interfering RNA demonstrated that the activation of p38 mitogen-activated protein kinase (MAPK) and phosphatidylinositol 3-kinase (PI3K)/Akt pathways are critical for SDF-1-induced uPA expression.	topic_ccc
74827	5	354955	7	NULL	NULL	0	NULL	PI3K	GP		is					phosphatidylinositol 3-kinase 	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	xperiments involving specific inhibitors and small interfering RNA demonstrated that the activation of p38 mitogen-activated protein kinase (MAPK) and phosphatidylinositol 3-kinase (PI3K)/Akt pathways are critical for SDF-1-induced uPA expression.	topic_ccc
74828	1	354956	7	NULL	NULL	0	NULL	DNA mismatch repair	Process		execute					5-fluorouracil	Chemical	cytotoxicity of			NULL	colorectal cancer cells	0	NULL	NULL	NULL	NULL	NULL	DNA mismatch repair proficiency executing 5-fluorouracil cytotoxicity in colorectal cancer cells.	topic_ccc
74829	1	354957	7	NULL	NULL	0	NULL	COX2 inhibitors	Chemical		widely used as					analgesics	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Selective cyclooxygenase-2 (COX2) inhibitors are widely used as analgesics and it is unclear whether its long-term use affects cancer risk	topic_ccc
74830	2	354957	7	NULL	NULL	0	NULL	COX2	GP		is					cyclooxygenase-2	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Selective cyclooxygenase-2 (COX2) inhibitors are widely used as analgesics and it is unclear whether its long-term use affects cancer risk	topic_ccc
74831	1	354958	7	NULL	NULL	0	NULL	SCN5A gene	GP		encode		specifically			VGSC isotype Na(v)1.5	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically, the SCN5A gene encoding the VGSC isotype Na(v)1.5 has been defined as a key driver of human cancer cell invasion.	topic_ccc
74832	2	354958	7	NULL	NULL	0	NULL	VGSC isotype Na(v)1.5	GP		key driver of					cancer cell 	cell	human;;invasion of			NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically, the SCN5A gene encoding the VGSC isotype Na(v)1.5 has been defined as a key driver of human cancer cell invasion.	topic_ccc
74833	1	354959	7	NULL	NULL	0	NULL	 COX2 inhibitors	Chemical	prolonged use of	increase					breast cancer	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged use of COX2 inhibitors was associated with an increased risk of breast and haematological cancers and decreased risk of colorectal cancer.	topic_ccc
74834	2	354959	7	NULL	NULL	NULL	NULL	COX2 inhibitors	Chemical	prolonged use of	increase					haematological cancers 	MedicalFinding	risk of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Prolonged use of COX2 inhibitors was associated with an increased risk of breast and haematological cancers and decreased risk of colorectal cancer.	topic_ccc
74835	3	354959	7	NULL	NULL	0	NULL	COX2 inhibitors	Chemical	prolonged use of	decrease					colorectal cancer	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged use of COX2 inhibitors was associated with an increased risk of breast and haematological cancers and decreased risk of colorectal cancer.	topic_ccc
74836	1	354961	7	NULL	NULL	0	NULL	fibroblast	Cell		synthesizes					extracellular matrix	CellComponent				NULL		0	NULL	NULL	NULL	NULL	NULL	A fibroblast is a type of cell that synthesizes the extracellular matrix and collagen,[1] the structural framework (stroma) for animal tissues, and plays a critical role in wound healing. 	topic_ccc
74837	2	354961	7	NULL	NULL	0	NULL	fibroblast	Cell		synthesizes					collagen	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	A fibroblast is a type of cell that synthesizes the extracellular matrix and collagen,[1] the structural framework (stroma) for animal tissues, and plays a critical role in wound healing. 	topic_ccc
74838	3	354961	7	NULL	NULL	NULL	NULL	collagen	GP		stroma for					animal tissues	OrganismPart				NULL		NULL	NULL	NULL	NULL	NULL	NULL	A fibroblast is a type of cell that synthesizes the extracellular matrix and collagen,[1] the structural framework (stroma) for animal tissues, and plays a critical role in wound healing. 	topic_ccc
74839	4	354961	7	NULL	NULL	0	NULL	collagen	GP		play a critical role in					wound healing	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	A fibroblast is a type of cell that synthesizes the extracellular matrix and collagen,[1] the structural framework (stroma) for animal tissues, and plays a critical role in wound healing. 	topic_ccc
74845	5	354961	7	NULL	NULL	0	NULL	stroma	GP		is					structural framework	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	A fibroblast is a type of cell that synthesizes the extracellular matrix and collagen,[1] the structural framework (stroma) for animal tissues, and plays a critical role in wound healing. 	topic_ccc
74840	1	354962	7	NULL	NULL	0	NULL	sporadic colorectal cancer	MedicalFinding		characterized by					microsatellite sequences	NucleicAcid	mutations in			NULL		0	NULL	NULL	NULL	NULL	NULL	This pathway is present in nearly 15% of all cases of sporadic colorectal cancer. It is characterized by the presence of mutations in the microsatellite sequences caused by a defect in the DNA mismatch repair genes, mostly in hMLH1 or hMSH2.	topic_ccc
74841	2	354962	7	NULL	NULL	0	NULL	microsatellite sequences	NucleicAcid	mutations in	caused by					hMLH1	GP	defect in			NULL		0	NULL	NULL	NULL	NULL	NULL	This pathway is present in nearly 15% of all cases of sporadic colorectal cancer. It is characterized by the presence of mutations in the microsatellite sequences caused by a defect in the DNA mismatch repair genes, mostly in hMLH1 or hMSH2.	topic_ccc
74842	3	354962	7	NULL	NULL	0	NULL	 microsatellite sequences	NucleicAcid	mutations in	caused by					hMSH2	GP	defect in			NULL		0	NULL	NULL	NULL	NULL	NULL	This pathway is present in nearly 15% of all cases of sporadic colorectal cancer. It is characterized by the presence of mutations in the microsatellite sequences caused by a defect in the DNA mismatch repair genes, mostly in hMLH1 or hMSH2.	topic_ccc
74843	4	354962	7	NULL	NULL	0	NULL	hMLH1	GP		is a type of					DNA mismatch repair genes	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	This pathway is present in nearly 15% of all cases of sporadic colorectal cancer. It is characterized by the presence of mutations in the microsatellite sequences caused by a defect in the DNA mismatch repair genes, mostly in hMLH1 or hMSH2.	topic_ccc
74844	5	354962	7	NULL	NULL	0	NULL	hMSH2	GP		is a type of					DNA mismatch repair genes	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	This pathway is present in nearly 15% of all cases of sporadic colorectal cancer. It is characterized by the presence of mutations in the microsatellite sequences caused by a defect in the DNA mismatch repair genes, mostly in hMLH1 or hMSH2.	topic_ccc
74846	1	354963	7	NULL	NULL	0	NULL	LS	MedicalFinding		caused by					MSH2	GP	germline mutations in			NULL		0	NULL	NULL	NULL	NULL	NULL	Lynch syndrome (LS) is caused by germline mutations in MSH2, MLH1, MSH6, and PMS2 mismatch-repair genes and leads to a high risk of colorectal and endometrial cancer.	topic_ccc
74847	2	354963	7	NULL	NULL	0	NULL	LS	MedicalFinding		caused by					MLH1	GP	germline mutations in			NULL		0	NULL	NULL	NULL	NULL	NULL	Lynch syndrome (LS) is caused by germline mutations in MSH2, MLH1, MSH6, and PMS2 mismatch-repair genes and leads to a high risk of colorectal and endometrial cancer.	topic_ccc
74848	3	354963	7	NULL	NULL	0	NULL	LS	MedicalFinding		caused by					PMS2 mismatch-repair genes	GP	germline mutations in			NULL		0	NULL	NULL	NULL	NULL	NULL	Lynch syndrome (LS) is caused by germline mutations in MSH2, MLH1, MSH6, and PMS2 mismatch-repair genes and leads to a high risk of colorectal and endometrial cancer.	topic_ccc
74849	4	354963	7	NULL	NULL	0	NULL	LS	MedicalFinding		leads to					colorectal cancer	MedicalFinding	high risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	Lynch syndrome (LS) is caused by germline mutations in MSH2, MLH1, MSH6, and PMS2 mismatch-repair genes and leads to a high risk of colorectal and endometrial cancer.	topic_ccc
74850	5	354963	7	NULL	NULL	NULL	NULL	LS	MedicalFinding		leads to					endometrial cancer	MedicalFinding	high risk of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Lynch syndrome (LS) is caused by germline mutations in MSH2, MLH1, MSH6, and PMS2 mismatch-repair genes and leads to a high risk of colorectal and endometrial cancer.	topic_ccc
74851	7	354963	7	NULL	NULL	NULL	NULL	LS	MedicalFinding		is					Lynch syndrome	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Lynch syndrome (LS) is caused by germline mutations in MSH2, MLH1, MSH6, and PMS2 mismatch-repair genes and leads to a high risk of colorectal and endometrial cancer.	topic_ccc
74852	8	354963	7	NULL	NULL	0	NULL	LS	MedicalFinding		caused by					MSH6	GP	germline mutations in			NULL		0	NULL	NULL	NULL	NULL	NULL	Lynch syndrome (LS) is caused by germline mutations in MSH2, MLH1, MSH6, and PMS2 mismatch-repair genes and leads to a high risk of colorectal and endometrial cancer.	topic_ccc
74854	1	354966	7	NULL	NULL	0	NULL	MMR	Process		due to					hMLH-1	GP	hypermethylation of		promoter	NULL		0	NULL	NULL	NULL	NULL	NULL	In sporadic CRCs, MMR is usually due to hypermethylation of the hMLH-1 promoter. 	topic_ccc
74855	2	354966	7	NULL	NULL	0	NULL	statement 1	Process		occur in					sporadic CRCs	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In sporadic CRCs, MMR is usually due to hypermethylation of the hMLH-1 promoter. 	topic_ccc
74876	1	354967	7	NULL	NULL	0	NULL	APC gene	GP	mutation of	congenital in					FAP syndrome	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The APC gene can be mutated in several ways during the colonic oncogenesis: congenital in the FAP syndrome, somatic in sporadic colorectal cancers and secondary to the MYH gene inactivation in MAP syndrome.	topic_ccc
74877	2	354967	7	NULL	NULL	0	NULL	APC gene	GP	somatic mutation of	occur in					sporadic colorectal cancers	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The APC gene can be mutated in several ways during the colonic oncogenesis: congenital in the FAP syndrome, somatic in sporadic colorectal cancers and secondary to the MYH gene inactivation in MAP syndrome.	topic_ccc
74878	3	354967	7	NULL	NULL	NULL	NULL	APC gene	GP	mutation of	occur 					MYH gene	GP	secondary to inactivation of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	The APC gene can be mutated in several ways during the colonic oncogenesis: congenital in the FAP syndrome, somatic in sporadic colorectal cancers and secondary to the MYH gene inactivation in MAP syndrome.	topic_ccc
74879	4	354967	7	NULL	NULL	0	NULL	statement 3	Process		occur in					MAP syndrome	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The APC gene can be mutated in several ways during the colonic oncogenesis: congenital in the FAP syndrome, somatic in sporadic colorectal cancers and secondary to the MYH gene inactivation in MAP syndrome.	topic_ccc
74880	1	354969	7	NULL	NULL	0	NULL	MMR	Process	inactivation of	result in					RER+ phenotype	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	NULL	NULL	These changes result in MMR inactivation, which causes RER+ phenotype. Our results suggest a connection between alteration in some tumor suppressor genes and MSI phenotype of sporadic colorectal cancer in Bosnian population.	topic_ccc
74881	2	354969	7	NULL	NULL	0	NULL	tumor suppressor genes	GP	alteration in	connected to					MSI phenotype 	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	NULL	NULL	These changes result in MMR inactivation, which causes RER+ phenotype. Our results suggest a connection between alteration in some tumor suppressor genes and MSI phenotype of sporadic colorectal cancer in Bosnian population.	topic_ccc
74882	3	354969	7	NULL	NULL	0	NULL	statement 2	Process		occur in					sporadic colorectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	These changes result in MMR inactivation, which causes RER+ phenotype. Our results suggest a connection between alteration in some tumor suppressor genes and MSI phenotype of sporadic colorectal cancer in Bosnian population.	topic_ccc
74883	4	354969	7	NULL	NULL	0	NULL	statement 2	Process		occur in					Bosnian population	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	These changes result in MMR inactivation, which causes RER+ phenotype. Our results suggest a connection between alteration in some tumor suppressor genes and MSI phenotype of sporadic colorectal cancer in Bosnian population.	topic_ccc
74924	1	354970	7	NULL	NULL	0	NULL	IL-8	GP	overexpression of	promotes					tumor growth	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Together, these findings indicate that overexpression of IL-8 promotes tumor growth, metastasis, chemoresistance and angiogenesis, implying IL-8 to be an important therapeutic target in CRC.	topic_ccc
74925	2	354970	7	NULL	NULL	0	NULL	IL-8	GP	overexpression of	promotes					metastasis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Together, these findings indicate that overexpression of IL-8 promotes tumor growth, metastasis, chemoresistance and angiogenesis, implying IL-8 to be an important therapeutic target in CRC.	topic_ccc
74926	3	354970	7	NULL	NULL	0	NULL	IL-8	GP	overexpression of	promotes					chemoresistance	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Together, these findings indicate that overexpression of IL-8 promotes tumor growth, metastasis, chemoresistance and angiogenesis, implying IL-8 to be an important therapeutic target in CRC.	topic_ccc
74927	4	354970	7	NULL	NULL	0	NULL	 IL-8	GP	overexpression of	promotes					angiogenesis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Together, these findings indicate that overexpression of IL-8 promotes tumor growth, metastasis, chemoresistance and angiogenesis, implying IL-8 to be an important therapeutic target in CRC.	topic_ccc
74928	5	354970	7	NULL	NULL	0	NULL	IL-8	GP		therapeutic target in					CRC	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Together, these findings indicate that overexpression of IL-8 promotes tumor growth, metastasis, chemoresistance and angiogenesis, implying IL-8 to be an important therapeutic target in CRC.	topic_ccc
74929	6	354970	7	NULL	NULL	0	NULL	statement 1	Process		implies					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Together, these findings indicate that overexpression of IL-8 promotes tumor growth, metastasis, chemoresistance and angiogenesis, implying IL-8 to be an important therapeutic target in CRC.	topic_ccc
74930	7	354970	7	NULL	NULL	0	NULL	statement 2	Process		implies					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Together, these findings indicate that overexpression of IL-8 promotes tumor growth, metastasis, chemoresistance and angiogenesis, implying IL-8 to be an important therapeutic target in CRC.	topic_ccc
74938	8	354970	7	NULL	NULL	0	NULL	statement 3	Process		implies					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Together, these findings indicate that overexpression of IL-8 promotes tumor growth, metastasis, chemoresistance and angiogenesis, implying IL-8 to be an important therapeutic target in CRC.	topic_ccc
74939	9	354970	7	NULL	NULL	0	NULL	statement 4	Process		implies					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Together, these findings indicate that overexpression of IL-8 promotes tumor growth, metastasis, chemoresistance and angiogenesis, implying IL-8 to be an important therapeutic target in CRC.	topic_ccc
74940	1	354972	7	NULL	NULL	0	NULL	IL-8	GP		is a type of					chemokine	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-8 (IL-8), a chemokine with a defining CXC amino acid motif, is known to possess tumorigenic and proangiogenic properties. Overexpression of IL-8 has been detected in many human tumors, including colorectal cancer (CRC), and is associated with poor prognosis.	topic_ccc
74941	2	354972	7	NULL	NULL	0	NULL	IL-8	GP		possess			CXC amino acid motif		tumorigenic properties	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-8 (IL-8), a chemokine with a defining CXC amino acid motif, is known to possess tumorigenic and proangiogenic properties. Overexpression of IL-8 has been detected in many human tumors, including colorectal cancer (CRC), and is associated with poor prognosis.	topic_ccc
74942	3	354972	7	NULL	NULL	0	NULL	IL-8	GP		possess			CXC amino acid motif		proangiogenic properties	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-8 (IL-8), a chemokine with a defining CXC amino acid motif, is known to possess tumorigenic and proangiogenic properties. Overexpression of IL-8 has been detected in many human tumors, including colorectal cancer (CRC), and is associated with poor prognosis.	topic_ccc
74943	4	354972	7	NULL	NULL	0	NULL	IL-8	GP	overexpression of	is detected in					CRC	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-8 (IL-8), a chemokine with a defining CXC amino acid motif, is known to possess tumorigenic and proangiogenic properties. Overexpression of IL-8 has been detected in many human tumors, including colorectal cancer (CRC), and is associated with poor prognosis.	topic_ccc
74944	5	354972	7	NULL	NULL	0	NULL	IL-8	GP	overexpression of	is associated with					CRC	MedicalFinding	poor prognosis of			NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-8 (IL-8), a chemokine with a defining CXC amino acid motif, is known to possess tumorigenic and proangiogenic properties. Overexpression of IL-8 has been detected in many human tumors, including colorectal cancer (CRC), and is associated with poor prognosis.	topic_ccc
74945	6	354972	7	NULL	NULL	0	NULL	CRC	MedicalFinding		is					colorectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-8 (IL-8), a chemokine with a defining CXC amino acid motif, is known to possess tumorigenic and proangiogenic properties. Overexpression of IL-8 has been detected in many human tumors, including colorectal cancer (CRC), and is associated with poor prognosis.	topic_ccc
74946	7	354972	7	NULL	NULL	0	NULL	CRC	MedicalFinding		is a type of					human tumor	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-8 (IL-8), a chemokine with a defining CXC amino acid motif, is known to possess tumorigenic and proangiogenic properties. Overexpression of IL-8 has been detected in many human tumors, including colorectal cancer (CRC), and is associated with poor prognosis.	topic_ccc
74947	8	354972	7	NULL	NULL	0	NULL	IL-8	GP		is					Interleukin-8	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-8 (IL-8), a chemokine with a defining CXC amino acid motif, is known to possess tumorigenic and proangiogenic properties. Overexpression of IL-8 has been detected in many human tumors, including colorectal cancer (CRC), and is associated with poor prognosis.	topic_ccc
74948	1	354973	7	NULL	NULL	0	NULL	 IL-8	GP	overexpression of	is detected in					CRC	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of IL-8 has been detected in many human tumors, including colorectal cancer (CRC), and is associated with poor prognosis.	topic_ccc
74949	2	354973	7	NULL	NULL	0	NULL	CRC	MedicalFinding		is					colorectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of IL-8 has been detected in many human tumors, including colorectal cancer (CRC), and is associated with poor prognosis.	topic_ccc
74950	3	354973	7	NULL	NULL	0	NULL	CRC	MedicalFinding		is a type of					human tumor	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of IL-8 has been detected in many human tumors, including colorectal cancer (CRC), and is associated with poor prognosis.	topic_ccc
74951	4	354973	7	NULL	NULL	0	NULL	IL-8	GP	overexpression of	is associated with					CRC	MedicalFinding	poor prognosis of			NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of IL-8 has been detected in many human tumors, including colorectal cancer (CRC), and is associated with poor prognosis.	topic_ccc
74952	1	354974	7	NULL	NULL	0	NULL	IL-8	GP		is a type of					chemokine	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-8 (IL-8), a chemokine with a defining CXC amino acid motif, is known to possess tumorigenic and proangiogenic properties.	topic_ccc
74953	2	354974	7	NULL	NULL	0	NULL	IL-8	GP		possess			CXC amino acid motif		tumorigenic properties	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-8 (IL-8), a chemokine with a defining CXC amino acid motif, is known to possess tumorigenic and proangiogenic properties.	topic_ccc
74954	3	354974	7	NULL	NULL	0	NULL	IL-8	GP		possess			CXC amino acid motif		proangiogenic properties	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-8 (IL-8), a chemokine with a defining CXC amino acid motif, is known to possess tumorigenic and proangiogenic properties.	topic_ccc
74955	4	354974	7	NULL	NULL	0	NULL	IL-8	GP		is					Interleukin-8	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-8 (IL-8), a chemokine with a defining CXC amino acid motif, is known to possess tumorigenic and proangiogenic properties.	topic_ccc
74956	1	354975	7	NULL	NULL	0	NULL	 IL-8	GP	overexpression of	is detected in					CRC	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of IL-8 has been detected in many human tumors, including colorectal cancer (CRC). The IL-8 transfectants demonstrated increased cellular proliferation.	topic_ccc
74957	2	354975	7	NULL	NULL	0	NULL	CRC	MedicalFinding		is a type of					human tumor	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of IL-8 has been detected in many human tumors, including colorectal cancer (CRC). The IL-8 transfectants demonstrated increased cellular proliferation.	topic_ccc
74958	3	354975	7	NULL	NULL	0	NULL	CRC	MedicalFinding		is					 colorectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of IL-8 has been detected in many human tumors, including colorectal cancer (CRC). The IL-8 transfectants demonstrated increased cellular proliferation.	topic_ccc
74959	1	354976	7	NULL	NULL	0	NULL	VGSC SCN5A	GP		 regulator of		high level			colon cancer invasion network	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Probabilistic modeling of loss-of-function screens and microarray data established an unequivocal role of VGSC SCN5A as a high level regulator of a colon cancer invasion network, involving genes that encompass Wnt signaling, cell migration, ectoderm development, response to biotic stimulus, steroid metabolic process, and cell cycle control.	topic_ccc
74960	2	354976	7	NULL	NULL	0	NULL	statement 1	Process		encompass					Wnt signaling	Process	genes involved in			NULL		0	NULL	NULL	NULL	NULL	NULL	Probabilistic modeling of loss-of-function screens and microarray data established an unequivocal role of VGSC SCN5A as a high level regulator of a colon cancer invasion network, involving genes that encompass Wnt signaling, cell migration, ectoderm development, response to biotic stimulus, steroid metabolic process, and cell cycle control.	topic_ccc
74961	3	354976	7	NULL	NULL	0	NULL	statement 1	Process		encompass					cell migration	Process	genes involved in			NULL		0	NULL	NULL	NULL	NULL	NULL	Probabilistic modeling of loss-of-function screens and microarray data established an unequivocal role of VGSC SCN5A as a high level regulator of a colon cancer invasion network, involving genes that encompass Wnt signaling, cell migration, ectoderm development, response to biotic stimulus, steroid metabolic process, and cell cycle control.	topic_ccc
74962	4	354976	7	NULL	NULL	0	NULL	statement 1	Process		encompass					ectoderm development	Process	genes involved in			NULL		0	NULL	NULL	NULL	NULL	NULL	Probabilistic modeling of loss-of-function screens and microarray data established an unequivocal role of VGSC SCN5A as a high level regulator of a colon cancer invasion network, involving genes that encompass Wnt signaling, cell migration, ectoderm development, response to biotic stimulus, steroid metabolic process, and cell cycle control.	topic_ccc
74963	5	354976	7	NULL	NULL	0	NULL	statement 1	Process		encompass					biotic stimulus	GP	genes involved in response to			NULL		0	NULL	NULL	NULL	NULL	NULL	Probabilistic modeling of loss-of-function screens and microarray data established an unequivocal role of VGSC SCN5A as a high level regulator of a colon cancer invasion network, involving genes that encompass Wnt signaling, cell migration, ectoderm development, response to biotic stimulus, steroid metabolic process, and cell cycle control.	topic_ccc
74964	6	354976	7	NULL	NULL	0	NULL	statement 1	Process		encompass					steroid metabolic process	Process	genes involved in			NULL		0	NULL	NULL	NULL	NULL	NULL	Probabilistic modeling of loss-of-function screens and microarray data established an unequivocal role of VGSC SCN5A as a high level regulator of a colon cancer invasion network, involving genes that encompass Wnt signaling, cell migration, ectoderm development, response to biotic stimulus, steroid metabolic process, and cell cycle control.	topic_ccc
74965	7	354976	7	NULL	NULL	0	NULL	statement 1	Process		encompass					cell cycle control	Process	genes involved in			NULL		0	NULL	NULL	NULL	NULL	NULL	Probabilistic modeling of loss-of-function screens and microarray data established an unequivocal role of VGSC SCN5A as a high level regulator of a colon cancer invasion network, involving genes that encompass Wnt signaling, cell migration, ectoderm development, response to biotic stimulus, steroid metabolic process, and cell cycle control.	topic_ccc
74999	1	354977	7	NULL	NULL	0	NULL	 network connectivity	Process		drives					colon cancer invasion	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	siRNA-mediated knockdown of predicted downstream network components caused a loss of invasive behavior, demonstrating network connectivity and its function in driving colon cancer invasion.	topic_ccc
75010	1	354979	7	NULL	NULL	0	NULL	VGSC	GP		mediates					invasive potential	QuantityOrMeasure				NULL		0	NULL	NULL	NULL	NULL	NULL	We explored the mechanism of VGSC-mediated invasive potential on the basis of reported links between VGSC activity and gene expression in excitable cells.	topic_ccc
75011	2	354979	7	NULL	NULL	0	NULL	VGSC activity	Process		linked to					gene expression	GP				NULL	excitable cells	0	NULL	NULL	NULL	NULL	NULL	We explored the mechanism of VGSC-mediated invasive potential on the basis of reported links between VGSC activity and gene expression in excitable cells.	topic_ccc
75012	1	354980	7	NULL	NULL	0	NULL	sulindac	Chemical		chemopreventive agent in					sporadic colorectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The non-steroidal anti-inflammatory drug sulindac is an effective chemopreventive agent in sporadic colorectal cancer but its potential benefit in mismatch repair deficient cancers remains to be defined.	topic_ccc
75013	2	354980	7	NULL	NULL	0	NULL	sulindac	Chemical		is a type of					non-steroidal anti-inflammatory drug	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The non-steroidal anti-inflammatory drug sulindac is an effective chemopreventive agent in sporadic colorectal cancer but its potential benefit in mismatch repair deficient cancers remains to be defined.	topic_ccc
75051	1	354981	7	NULL	NULL	0	NULL	SOX17	GP	restoration of	inhibit					HepG2 colony formation	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 Restoration of SOX17 inhibits HepG2 colony formation and β-catenin/TCF-dependent transcription with the presence of HMG box in SOX17.	topic_ccc
75052	2	354981	7	NULL	NULL	0	NULL	 transcription	Process		depends on					 β-catenin	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 Restoration of SOX17 inhibits HepG2 colony formation and β-catenin/TCF-dependent transcription with the presence of HMG box in SOX17.	topic_ccc
75053	3	354981	7	NULL	NULL	0	NULL	transcription	Process		depends on					TCF	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 Restoration of SOX17 inhibits HepG2 colony formation and β-catenin/TCF-dependent transcription with the presence of HMG box in SOX17.	topic_ccc
75054	4	354981	7	NULL	NULL	0	NULL	SOX17	GP	restoration of	inhibit					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 Restoration of SOX17 inhibits HepG2 colony formation and β-catenin/TCF-dependent transcription with the presence of HMG box in SOX17.	topic_ccc
75055	5	354981	7	NULL	NULL	0	NULL	SOX17	GP	restoration of	inhibit					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 Restoration of SOX17 inhibits HepG2 colony formation and β-catenin/TCF-dependent transcription with the presence of HMG box in SOX17.	topic_ccc
75056	6	354981	7	NULL	NULL	NULL	NULL	statement 4	Process		in the presence of					SOX17	GP		HMG box		NULL		NULL	NULL	NULL	NULL	NULL	NULL	 Restoration of SOX17 inhibits HepG2 colony formation and β-catenin/TCF-dependent transcription with the presence of HMG box in SOX17.	topic_ccc
75057	7	354981	7	NULL	NULL	NULL	NULL	statement 5	Process		in the presence of					SOX17	GP		HMG box		NULL		NULL	NULL	NULL	NULL	NULL	NULL	 Restoration of SOX17 inhibits HepG2 colony formation and β-catenin/TCF-dependent transcription with the presence of HMG box in SOX17.	topic_ccc
75059	1	354982	7	NULL	NULL	0	NULL	IL-12 	GP		displays					antitumor properties	Process				NULL	murine models of tumorigenesis	0	NULL	NULL	NULL	NULL	NULL	Moreover, in murine models of tumorigenesis, IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells. Importantly, IL-12 through IFN- γ -dependent induction of the antiangiogenic factors interferon-inducible protein (IP) 10 and monokine induced by gamma interferon (MIG) contributes to tumor eradication. 	topic_ccc
75060	2	354982	7	NULL	NULL	0	NULL	CD4+ cells	Cell		secrete					(IFN)-γ 	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, in murine models of tumorigenesis, IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells. Importantly, IL-12 through IFN- γ -dependent induction of the antiangiogenic factors interferon-inducible protein (IP) 10 and monokine induced by gamma interferon (MIG) contributes to tumor eradication. 	topic_ccc
75061	3	354982	7	NULL	NULL	0	NULL	CD8+ T cells	Cell		secrete					(IFN)-γ	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, in murine models of tumorigenesis, IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells. Importantly, IL-12 through IFN- γ -dependent induction of the antiangiogenic factors interferon-inducible protein (IP) 10 and monokine induced by gamma interferon (MIG) contributes to tumor eradication. 	topic_ccc
75062	4	354982	7	NULL	NULL	0	NULL	NK cells	Cell		secrete					(IFN)-γ	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, in murine models of tumorigenesis, IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells. Importantly, IL-12 through IFN- γ -dependent induction of the antiangiogenic factors interferon-inducible protein (IP) 10 and monokine induced by gamma interferon (MIG) contributes to tumor eradication. 	topic_ccc
75063	5	354982	7	NULL	NULL	0	NULL	NK-T cells	Cell		secrete					(IFN)-γ	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, in murine models of tumorigenesis, IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells. Importantly, IL-12 through IFN- γ -dependent induction of the antiangiogenic factors interferon-inducible protein (IP) 10 and monokine induced by gamma interferon (MIG) contributes to tumor eradication. 	topic_ccc
75064	6	354982	7	NULL	NULL	0	NULL	statement 1	Process		mediated by		mainly			statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, in murine models of tumorigenesis, IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells. Importantly, IL-12 through IFN- γ -dependent induction of the antiangiogenic factors interferon-inducible protein (IP) 10 and monokine induced by gamma interferon (MIG) contributes to tumor eradication. 	topic_ccc
75065	7	354982	7	NULL	NULL	0	NULL	statement 1	Process		mediated by		mainly			statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, in murine models of tumorigenesis, IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells. Importantly, IL-12 through IFN- γ -dependent induction of the antiangiogenic factors interferon-inducible protein (IP) 10 and monokine induced by gamma interferon (MIG) contributes to tumor eradication. 	topic_ccc
75066	8	354982	7	NULL	NULL	NULL	NULL	statement 1	Process		mediated by		mainly			statement 4	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Moreover, in murine models of tumorigenesis, IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells. Importantly, IL-12 through IFN- γ -dependent induction of the antiangiogenic factors interferon-inducible protein (IP) 10 and monokine induced by gamma interferon (MIG) contributes to tumor eradication. 	topic_ccc
75067	9	354982	7	NULL	NULL	0	NULL	statement 1	Process		mediated by		mainly			statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, in murine models of tumorigenesis, IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells. Importantly, IL-12 through IFN- γ -dependent induction of the antiangiogenic factors interferon-inducible protein (IP) 10 and monokine induced by gamma interferon (MIG) contributes to tumor eradication. 	topic_ccc
75068	10	354982	7	NULL	NULL	0	NULL	NK cells	cell		is					natural killer cells	cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, in murine models of tumorigenesis, IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells. Importantly, IL-12 through IFN- γ -dependent induction of the antiangiogenic factors interferon-inducible protein (IP) 10 and monokine induced by gamma interferon (MIG) contributes to tumor eradication. 	topic_ccc
75069	11	354982	7	NULL	NULL	0	NULL	 IL-12	GP		contributes to					tumor eradication	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, in murine models of tumorigenesis, IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells. Importantly, IL-12 through IFN- γ -dependent induction of the antiangiogenic factors interferon-inducible protein (IP) 10 and monokine induced by gamma interferon (MIG) contributes to tumor eradication. 	topic_ccc
75070	12	354982	7	NULL	NULL	0	NULL	IP 10	GP	induction of	depends on					IFN- γ	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, in murine models of tumorigenesis, IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells. Importantly, IL-12 through IFN- γ -dependent induction of the antiangiogenic factors interferon-inducible protein (IP) 10 and monokine induced by gamma interferon (MIG) contributes to tumor eradication. 	topic_ccc
75071	13	354982	7	NULL	NULL	0	NULL	gamma interferon 	GP		induce					monokine	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, in murine models of tumorigenesis, IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells. Importantly, IL-12 through IFN- γ -dependent induction of the antiangiogenic factors interferon-inducible protein (IP) 10 and monokine induced by gamma interferon (MIG) contributes to tumor eradication. 	topic_ccc
75072	14	354982	7	NULL	NULL	NULL	NULL	statement 11	Process		occur through					statement 12	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Moreover, in murine models of tumorigenesis, IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells. Importantly, IL-12 through IFN- γ -dependent induction of the antiangiogenic factors interferon-inducible protein (IP) 10 and monokine induced by gamma interferon (MIG) contributes to tumor eradication. 	topic_ccc
75073	15	354982	7	NULL	NULL	0	NULL	statement 11	Process		occur through					statement 13	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, in murine models of tumorigenesis, IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells. Importantly, IL-12 through IFN- γ -dependent induction of the antiangiogenic factors interferon-inducible protein (IP) 10 and monokine induced by gamma interferon (MIG) contributes to tumor eradication. 	topic_ccc
75074	16	354982	7	NULL	NULL	0	NULL	IP 10	GP		is a type of					 interferon-inducible protein 	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, in murine models of tumorigenesis, IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells. Importantly, IL-12 through IFN- γ -dependent induction of the antiangiogenic factors interferon-inducible protein (IP) 10 and monokine induced by gamma interferon (MIG) contributes to tumor eradication. 	topic_ccc
75075	17	354982	7	NULL	NULL	0	NULL	IP 10	GP		is a type of					antiangiogenic factors	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, in murine models of tumorigenesis, IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells. Importantly, IL-12 through IFN- γ -dependent induction of the antiangiogenic factors interferon-inducible protein (IP) 10 and monokine induced by gamma interferon (MIG) contributes to tumor eradication. 	topic_ccc
75076	18	354982	7	NULL	NULL	0	NULL	MIG	GP		is					monokine induced by gamma interferon 	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, in murine models of tumorigenesis, IL-12 displays remarkable antitumor properties that are mainly mediated by interferon (IFN)-γ secretion by CD4+, CD8+ T cells, natural killer (NK) or NK-T cells. Importantly, IL-12 through IFN- γ -dependent induction of the antiangiogenic factors interferon-inducible protein (IP) 10 and monokine induced by gamma interferon (MIG) contributes to tumor eradication. 	topic_ccc
75077	1	354983	7	NULL	NULL	NULL	NULL	S100A4 immunoreactivity protein	GP		absent in					cytoplasm	CellComponent				NULL	normal colorectal mucosa	NULL	NULL	NULL	NULL	NULL	NULL	In normal colorectal mucosa, protein S100A4 immunoreactivity was clearly absent in both cytoplasm and nucleus.	topic_ccc
75078	2	354983	7	NULL	NULL	0	NULL	S100A4 immunoreactivity protein	GP		absent in					nucleus	CellComponent				NULL	normal colorectal mucosa	0	NULL	NULL	NULL	NULL	NULL	In normal colorectal mucosa, protein S100A4 immunoreactivity was clearly absent in both cytoplasm and nucleus.	topic_ccc
75079	1	354985	7	NULL	NULL	0	NULL	Vitamin D	Chemical		is a group of					fat-soluble secosteroids	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Vitamin D is a group of fat-soluble secosteroids.	topic_ccc
75081	1	354987	7	NULL	NULL	NULL	NULL	Calcium 	Chemical		protect					polyps	MedicalFinding	high-risk people from developing			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Calcium seems to protect high-risk people from developing the polyps that can lead to colorectal cancer	topic_ccc
75082	2	354987	7	NULL	NULL	0	NULL	polyps	MedicalFinding		 lead to		could			colorectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Calcium seems to protect high-risk people from developing the polyps that can lead to colorectal cancer	topic_ccc
75083	1	354988	7	NULL	NULL	0	NULL	cigarette smoking 	PhysicalPhenomenon		play roles in					colorectal carcinogenesis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion, cigarette smoking and alcohol consumption play roles in colorectal carcinogenesis, and the association differs by the clinical features of the adenomas.	topic_ccc
75084	2	354988	7	NULL	NULL	0	NULL	alcohol consumption	PhysicalPhenomenon		play roles in					colorectal carcinogenesis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion, cigarette smoking and alcohol consumption play roles in colorectal carcinogenesis, and the association differs by the clinical features of the adenomas.	topic_ccc
75085	1	354989	7	NULL	NULL	0	NULL	bFGF	GP		mitogen for					endothelial cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Basic fibroblast growth factor (bFGF) is a mitogen for endothelial cells, which participates in tumor angiogenesis. In vitro, a CTL assay revealed that bFGF-specific cytotoxic T lymphocytes (CTL) resulted in the lysis of mouse microvascular endothelial cells (MS1) rather than that of the CT26 colorectal cancer cells.	topic_ccc
75086	2	354989	7	NULL	NULL	0	NULL	statement 1	Process		participates in					tumor angiogenesis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Basic fibroblast growth factor (bFGF) is a mitogen for endothelial cells, which participates in tumor angiogenesis. In vitro, a CTL assay revealed that bFGF-specific cytotoxic T lymphocytes (CTL) resulted in the lysis of mouse microvascular endothelial cells (MS1) rather than that of the CT26 colorectal cancer cells.	topic_ccc
75087	3	354989	7	NULL	NULL	NULL	NULL	bFGF-specific CTL	Cell		lyse					MS1	Cell	mouse			NULL	in vitro	NULL	NULL	NULL	NULL	NULL	NULL	Basic fibroblast growth factor (bFGF) is a mitogen for endothelial cells, which participates in tumor angiogenesis. In vitro, a CTL assay revealed that bFGF-specific cytotoxic T lymphocytes (CTL) resulted in the lysis of mouse microvascular endothelial cells (MS1) rather than that of the CT26 colorectal cancer cells.	topic_ccc
75088	4	354989	7	NULL	NULL	NULL	NULL	bFGF-specific CTL	Cell		does not lyse					CT26 colorectal cancer cells	Cell				NULL	in vitro	NULL	NULL	NULL	NULL	NULL	NULL	Basic fibroblast growth factor (bFGF) is a mitogen for endothelial cells, which participates in tumor angiogenesis. In vitro, a CTL assay revealed that bFGF-specific cytotoxic T lymphocytes (CTL) resulted in the lysis of mouse microvascular endothelial cells (MS1) rather than that of the CT26 colorectal cancer cells.	topic_ccc
75089	5	354989	7	NULL	NULL	0	NULL	bFGF	GP		is					Basic fibroblast growth factor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Basic fibroblast growth factor (bFGF) is a mitogen for endothelial cells, which participates in tumor angiogenesis. In vitro, a CTL assay revealed that bFGF-specific cytotoxic T lymphocytes (CTL) resulted in the lysis of mouse microvascular endothelial cells (MS1) rather than that of the CT26 colorectal cancer cells.	topic_ccc
75090	6	354989	7	NULL	NULL	0	NULL	CTL	Cell		is					cytotoxic T lymphocytes 	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Basic fibroblast growth factor (bFGF) is a mitogen for endothelial cells, which participates in tumor angiogenesis. In vitro, a CTL assay revealed that bFGF-specific cytotoxic T lymphocytes (CTL) resulted in the lysis of mouse microvascular endothelial cells (MS1) rather than that of the CT26 colorectal cancer cells.	topic_ccc
75091	7	354989	7	NULL	NULL	0	NULL	MS1	Cell		is					microvascular endothelial cells 	Cell	mouse			NULL		0	NULL	NULL	NULL	NULL	NULL	Basic fibroblast growth factor (bFGF) is a mitogen for endothelial cells, which participates in tumor angiogenesis. In vitro, a CTL assay revealed that bFGF-specific cytotoxic T lymphocytes (CTL) resulted in the lysis of mouse microvascular endothelial cells (MS1) rather than that of the CT26 colorectal cancer cells.	topic_ccc
75092	1	354994	7	NULL	NULL	0	NULL	VEGF	GP		possess					angiogenic mechanism	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the association of serum levels of proangiogenic cytokines with different indices of social support and loneliness by measuring the levels of expression of two important proangiogenic cytokines, vascular endothelial growth factor (VEGF), and interleukin-6 in tumors of colon and rectum.The results of this study suggest VEGF to be an angiogenic mechanism through which loneliness may lead to worse cancer-related outcomes.	topic_ccc
75093	2	354994	7	NULL	NULL	0	NULL	VEGF	GP		is					vascular endothelial growth factor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the association of serum levels of proangiogenic cytokines with different indices of social support and loneliness by measuring the levels of expression of two important proangiogenic cytokines, vascular endothelial growth factor (VEGF), and interleukin-6 in tumors of colon and rectum.The results of this study suggest VEGF to be an angiogenic mechanism through which loneliness may lead to worse cancer-related outcomes.	topic_ccc
75094	3	354994	7	NULL	NULL	0	NULL	loneliness	MentalProcess		leads to					cancer-related outcomes	MedicalFinding	worse			NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the association of serum levels of proangiogenic cytokines with different indices of social support and loneliness by measuring the levels of expression of two important proangiogenic cytokines, vascular endothelial growth factor (VEGF), and interleukin-6 in tumors of colon and rectum.The results of this study suggest VEGF to be an angiogenic mechanism through which loneliness may lead to worse cancer-related outcomes.	topic_ccc
75095	4	354994	7	NULL	NULL	0	NULL	VEGF	GP		is a type of					proangiogenic cytokines	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the association of serum levels of proangiogenic cytokines with different indices of social support and loneliness by measuring the levels of expression of two important proangiogenic cytokines, vascular endothelial growth factor (VEGF), and interleukin-6 in tumors of colon and rectum.The results of this study suggest VEGF to be an angiogenic mechanism through which loneliness may lead to worse cancer-related outcomes.	topic_ccc
75096	5	354994	7	NULL	NULL	0	NULL	interleukin-6	GP		is a type of					proangiogenic cytokines	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the association of serum levels of proangiogenic cytokines with different indices of social support and loneliness by measuring the levels of expression of two important proangiogenic cytokines, vascular endothelial growth factor (VEGF), and interleukin-6 in tumors of colon and rectum.The results of this study suggest VEGF to be an angiogenic mechanism through which loneliness may lead to worse cancer-related outcomes.	topic_ccc
75097	1	354995	7	NULL	NULL	0	NULL	CRC tumors	MedicalFinding		negative for					VEGFR2	GP	expression of			NULL		0	NULL	NULL	NULL	NULL	NULL	The authors have previously observed that up to 40% of vessels in colorectal carcinoma (CRC) tumors are negative for VEGF receptor 2 (VEGFR2) expression. Differential activity of transforming growth factor beta (TGF-β) is a potential contributor to this receptor heterogeneity because TGF-β contributes to both angiogenesis and CRC tumor progression.	topic_ccc
75098	2	354995	7	NULL	NULL	0	NULL	TGF-β	GP		potential contributor to					receptor heterogeneity	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The authors have previously observed that up to 40% of vessels in colorectal carcinoma (CRC) tumors are negative for VEGF receptor 2 (VEGFR2) expression. Differential activity of transforming growth factor beta (TGF-β) is a potential contributor to this receptor heterogeneity because TGF-β contributes to both angiogenesis and CRC tumor progression.	topic_ccc
75099	3	354995	7	NULL	NULL	0	NULL	TGF-β	GP		contributes to					angiogenesis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The authors have previously observed that up to 40% of vessels in colorectal carcinoma (CRC) tumors are negative for VEGF receptor 2 (VEGFR2) expression. Differential activity of transforming growth factor beta (TGF-β) is a potential contributor to this receptor heterogeneity because TGF-β contributes to both angiogenesis and CRC tumor progression.	topic_ccc
75100	4	354995	7	NULL	NULL	0	NULL	TGF-β	GP		contributes to					CRC tumor	MedicalFinding	progression of			NULL		0	NULL	NULL	NULL	NULL	NULL	The authors have previously observed that up to 40% of vessels in colorectal carcinoma (CRC) tumors are negative for VEGF receptor 2 (VEGFR2) expression. Differential activity of transforming growth factor beta (TGF-β) is a potential contributor to this receptor heterogeneity because TGF-β contributes to both angiogenesis and CRC tumor progression.	topic_ccc
75101	5	354995	7	NULL	NULL	0	NULL	CRC	MedicalFinding		is					 colorectal carcinoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The authors have previously observed that up to 40% of vessels in colorectal carcinoma (CRC) tumors are negative for VEGF receptor 2 (VEGFR2) expression. Differential activity of transforming growth factor beta (TGF-β) is a potential contributor to this receptor heterogeneity because TGF-β contributes to both angiogenesis and CRC tumor progression.	topic_ccc
75102	6	354995	7	NULL	NULL	0	NULL	VEGFR2	GP		is					VEGF receptor 2	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The authors have previously observed that up to 40% of vessels in colorectal carcinoma (CRC) tumors are negative for VEGF receptor 2 (VEGFR2) expression. Differential activity of transforming growth factor beta (TGF-β) is a potential contributor to this receptor heterogeneity because TGF-β contributes to both angiogenesis and CRC tumor progression.	topic_ccc
75103	1	354996	7	NULL	NULL	0	NULL	Peritoneal elastic laminal invasion 	Process		associated with					colon cancer	MedicalFinding	recurrence in			NULL		0	NULL	NULL	NULL	NULL	NULL	Peritoneal elastic laminal invasion was associated with recurrence and prognosis in colon cancer and was an independent risk factor for the recurrence of stage II colon cancer.	topic_ccc
75104	2	354996	7	NULL	NULL	0	NULL	Peritoneal elastic laminal invasion 	Process		associated with					colon cancer	MedicalFinding	prognosis in			NULL		0	NULL	NULL	NULL	NULL	NULL	Peritoneal elastic laminal invasion was associated with recurrence and prognosis in colon cancer and was an independent risk factor for the recurrence of stage II colon cancer.	topic_ccc
75105	3	354996	7	NULL	NULL	NULL	NULL	Peritoneal elastic laminal invasion 	Process		 risk factor for		independent			stage II colon cancer	MedicalFinding	recurrence of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Peritoneal elastic laminal invasion was associated with recurrence and prognosis in colon cancer and was an independent risk factor for the recurrence of stage II colon cancer.	topic_ccc
75106	1	354997	7	NULL	NULL	0	NULL	folate 	Chemical	low dietary	associated with					colorectal cancer	MedicalFinding	increased risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	Low dietary folate is associated with increased risk of colorectal cancer.	topic_ccc
75107	1	354998	7	NULL	NULL	0	NULL	Irinotecan	Chemical		used for					cancer	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	Irinotecan (Camptosar, Pfizer; Campto, Yakult Honsha) is a drug used for the treatment of cancer.Its main use is in colon cancer, in particular, in combination with other chemotherapy agents. Irinotecan is activated by hydrolysis to SN-38, an inhibitor of topoisomerase I.	topic_ccc
75108	2	354998	7	NULL	NULL	0	NULL	Irinotecan	Chemical		is used in the					colon cancer	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	Irinotecan (Camptosar, Pfizer; Campto, Yakult Honsha) is a drug used for the treatment of cancer.Its main use is in colon cancer, in particular, in combination with other chemotherapy agents. Irinotecan is activated by hydrolysis to SN-38, an inhibitor of topoisomerase I.	topic_ccc
75109	3	354998	7	NULL	NULL	0	NULL	Irinotecan	Chemical		hydrolyzed to					SN-38	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Irinotecan (Camptosar, Pfizer; Campto, Yakult Honsha) is a drug used for the treatment of cancer.Its main use is in colon cancer, in particular, in combination with other chemotherapy agents. Irinotecan is activated by hydrolysis to SN-38, an inhibitor of topoisomerase I.	topic_ccc
75110	4	354998	7	NULL	NULL	0	NULL	statement 3	Process		activates					Irinotecan	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Irinotecan (Camptosar, Pfizer; Campto, Yakult Honsha) is a drug used for the treatment of cancer.Its main use is in colon cancer, in particular, in combination with other chemotherapy agents. Irinotecan is activated by hydrolysis to SN-38, an inhibitor of topoisomerase I.	topic_ccc
75111	5	354998	7	NULL	NULL	0	NULL	SN-38	Chemical		inhibitor of					topoisomerase I	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Irinotecan (Camptosar, Pfizer; Campto, Yakult Honsha) is a drug used for the treatment of cancer.Its main use is in colon cancer, in particular, in combination with other chemotherapy agents. Irinotecan is activated by hydrolysis to SN-38, an inhibitor of topoisomerase I.	topic_ccc
75112	1	354999	7	NULL	NULL	0	NULL	Small bowel adenocarcinoma	MedicalFinding		diagnosed by					double balloon enteroscopy	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Small bowel adenocarcinoma diagnosed by double balloon enteroscopy in a patient with nonpolyposis colorectal cancer.	topic_ccc
75113	2	354999	7	NULL	NULL	0	NULL	statement 1	Process		done in					nonpolyposis colorectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Small bowel adenocarcinoma diagnosed by double balloon enteroscopy in a patient with nonpolyposis colorectal cancer.	topic_ccc
75114	1	355000	7	NULL	NULL	0	NULL	CRC	MedicalFinding		deadly form of		second most			cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Colorectal Cancer (CRC) is the second most deadly form of cancer among men and women, second to lung cancer.	topic_ccc
75115	2	355000	7	NULL	NULL	0	NULL	CRC	MedicalFinding		occur second to					lung cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Colorectal Cancer (CRC) is the second most deadly form of cancer among men and women, second to lung cancer.	topic_ccc
75116	3	355000	7	NULL	NULL	NULL	NULL	CRC	MedicalFinding		occur among					men	GroupOfPeople				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Colorectal Cancer (CRC) is the second most deadly form of cancer among men and women, second to lung cancer.	topic_ccc
75117	4	355000	7	NULL	NULL	0	NULL	CRC	MedicalFinding		occur among					women	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Colorectal Cancer (CRC) is the second most deadly form of cancer among men and women, second to lung cancer.	topic_ccc
75118	5	355000	7	NULL	NULL	0	NULL	CRC	MedicalFinding		is					Colorectal Cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Colorectal Cancer (CRC) is the second most deadly form of cancer among men and women, second to lung cancer.	topic_ccc
75119	1	355001	7	NULL	NULL	0	NULL	resected polyps 	MedicalFinding		is a type of					adenomatous	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	According to autopsy studies, colonic polyps occur in more than 30% of people over the age of 60. Approximately 70-80% of resected polyps are adenomatous. Adenomatous lesions have a well-documented relationship to colorectal cancer.	topic_ccc
75120	2	355001	7	NULL	NULL	0	NULL	Adenomatous lesions	MedicalFinding		relationship to					colorectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	According to autopsy studies, colonic polyps occur in more than 30% of people over the age of 60. Approximately 70-80% of resected polyps are adenomatous. Adenomatous lesions have a well-documented relationship to colorectal cancer.	topic_ccc
75121	1	355002	7	NULL	NULL	0	NULL	sulindac	Chemical		exert their		may			anti-neoplastic role	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 It may be stated that sulindac and celecoxib, the two NSAIDs may exert their anti-neoplastic role in colorectal cancer via modifying the physicochemical properties of the membranes.	topic_ccc
75122	2	355002	7	NULL	NULL	0	NULL	statement 1	Process		occur in					colorectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	 It may be stated that sulindac and celecoxib, the two NSAIDs may exert their anti-neoplastic role in colorectal cancer via modifying the physicochemical properties of the membranes.	topic_ccc
75123	3	355002	7	NULL	NULL	0	NULL	celecoxib	Chemical		exert their		may			anti-neoplastic role	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 It may be stated that sulindac and celecoxib, the two NSAIDs may exert their anti-neoplastic role in colorectal cancer via modifying the physicochemical properties of the membranes.	topic_ccc
75124	4	355002	7	NULL	NULL	0	NULL	statement 3	Process		occur in					colorectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	 It may be stated that sulindac and celecoxib, the two NSAIDs may exert their anti-neoplastic role in colorectal cancer via modifying the physicochemical properties of the membranes.	topic_ccc
75125	5	355002	7	NULL	NULL	0	NULL	statement 1	Process		via					membrane	CellComponent	modifying the physicochemical properties of			NULL		0	NULL	NULL	NULL	NULL	NULL	 It may be stated that sulindac and celecoxib, the two NSAIDs may exert their anti-neoplastic role in colorectal cancer via modifying the physicochemical properties of the membranes.	topic_ccc
75126	6	355002	7	NULL	NULL	0	NULL	statement 3	Process		via					membrane	CellComponent	modifying the physicochemical properties of			NULL		0	NULL	NULL	NULL	NULL	NULL	 It may be stated that sulindac and celecoxib, the two NSAIDs may exert their anti-neoplastic role in colorectal cancer via modifying the physicochemical properties of the membranes.	topic_ccc
75127	7	355002	7	NULL	NULL	0	NULL	sulindac	Chemical		is a type of					NSAID	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	 It may be stated that sulindac and celecoxib, the two NSAIDs may exert their anti-neoplastic role in colorectal cancer via modifying the physicochemical properties of the membranes.	topic_ccc
75128	8	355002	7	NULL	NULL	0	NULL	celecoxib	Chemical		is a type of					NSAID	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	 It may be stated that sulindac and celecoxib, the two NSAIDs may exert their anti-neoplastic role in colorectal cancer via modifying the physicochemical properties of the membranes.	topic_ccc
75129	1	355003	7	NULL	NULL	0	NULL	HIF-1α	GP		overexpressed in					human cancers	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous studies have shown that hypoxia-inducible factor 1α (HIF-1α) is overexpressed in many human cancers and up-regulates a host of hypoxia-responsive genes for cancer growth and survival.	topic_ccc
75130	2	355003	7	NULL	NULL	0	NULL	HIF-1α	GP		upregulate					hypoxia-responsive genes	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous studies have shown that hypoxia-inducible factor 1α (HIF-1α) is overexpressed in many human cancers and up-regulates a host of hypoxia-responsive genes for cancer growth and survival.	topic_ccc
75131	3	355003	7	NULL	NULL	0	NULL	hypoxia-responsive genes	GP		required for					cancer growth	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous studies have shown that hypoxia-inducible factor 1α (HIF-1α) is overexpressed in many human cancers and up-regulates a host of hypoxia-responsive genes for cancer growth and survival.	topic_ccc
75132	4	355003	7	NULL	NULL	0	NULL	hypoxia-responsive genes	GP		required for					cancer survival	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous studies have shown that hypoxia-inducible factor 1α (HIF-1α) is overexpressed in many human cancers and up-regulates a host of hypoxia-responsive genes for cancer growth and survival.	topic_ccc
75133	5	355003	7	NULL	NULL	0	NULL	HIF-1α	GP		is					 hypoxia-inducible factor 1α	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous studies have shown that hypoxia-inducible factor 1α (HIF-1α) is overexpressed in many human cancers and up-regulates a host of hypoxia-responsive genes for cancer growth and survival.	topic_ccc
75134	1	355004	7	NULL	NULL	0	NULL	HIF-1α			is linked to					angiogenesis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of hypoxia-inducible factor 1-alpha (HIF-1α), an important transcriptional factor linked with angiogenesis, was significantly down-regulated post 24 h hypoxia, HIF-1α expression could be significantly up-regulated and HIF-1α nuclear translocation significantly enhanced by pretreatment with GDF-15 in hypoxic HUVECs.	topic_ccc
75135	2	355004	7	NULL	NULL	0	NULL	statement 1	Process		down-regulated in		significantly			hypoxia	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of hypoxia-inducible factor 1-alpha (HIF-1α), an important transcriptional factor linked with angiogenesis, was significantly down-regulated post 24 h hypoxia, HIF-1α expression could be significantly up-regulated and HIF-1α nuclear translocation significantly enhanced by pretreatment with GDF-15 in hypoxic HUVECs.	topic_ccc
75136	3	355004	7	NULL	NULL	NULL	NULL	HIF-1α	GP	expression of	up-regulated by		significantly			GDF-15	Chemical	pretreatment with			NULL	hypoxic HUVECs	NULL	NULL	NULL	NULL	NULL	NULL	Expression of hypoxia-inducible factor 1-alpha (HIF-1α), an important transcriptional factor linked with angiogenesis, was significantly down-regulated post 24 h hypoxia, HIF-1α expression could be significantly up-regulated and HIF-1α nuclear translocation significantly enhanced by pretreatment with GDF-15 in hypoxic HUVECs.	topic_ccc
75137	4	355004	7	NULL	NULL	0	NULL	HIF-1α	GP	nuclear translocation of	enhanced by		significantly			GDF-15	Chemical	pretreatment with			NULL	hypoxic HUVECs	0	NULL	NULL	NULL	NULL	NULL	Expression of hypoxia-inducible factor 1-alpha (HIF-1α), an important transcriptional factor linked with angiogenesis, was significantly down-regulated post 24 h hypoxia, HIF-1α expression could be significantly up-regulated and HIF-1α nuclear translocation significantly enhanced by pretreatment with GDF-15 in hypoxic HUVECs.	topic_ccc
75138	5	355004	7	NULL	NULL	0	NULL	HIF-1α	GP		is					hypoxia-inducible factor 1-alpha	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of hypoxia-inducible factor 1-alpha (HIF-1α), an important transcriptional factor linked with angiogenesis, was significantly down-regulated post 24 h hypoxia, HIF-1α expression could be significantly up-regulated and HIF-1α nuclear translocation significantly enhanced by pretreatment with GDF-15 in hypoxic HUVECs.	topic_ccc
75139	6	355004	7	NULL	NULL	0	NULL	HIF-1α	GP		is a type of					transcriptional factor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of hypoxia-inducible factor 1-alpha (HIF-1α), an important transcriptional factor linked with angiogenesis, was significantly down-regulated post 24 h hypoxia, HIF-1α expression could be significantly up-regulated and HIF-1α nuclear translocation significantly enhanced by pretreatment with GDF-15 in hypoxic HUVECs.	topic_ccc
75140	1	355005	7	NULL	NULL	0	NULL	hepatic resection 	MedicalFinding	complications of extensive	encountered in					liver metastases 	Process	patients with			NULL		0	NULL	NULL	NULL	NULL	NULL	More and more complications of extensive hepatic resection are being encountered in patients treated for liver metastases from colorectal cancer.	topic_ccc
75141	2	355005	7	NULL	NULL	0	NULL	statement 1	Process		occur in					colorectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	More and more complications of extensive hepatic resection are being encountered in patients treated for liver metastases from colorectal cancer.	topic_ccc
75142	1	355006	7	NULL	NULL	0	NULL	COX-1	GP		expressed in		constitutively 			normal tissue	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	COX-1 is constitutively expressed in normal tissue, serving an important role in tissue homeostasis, whereas COX-2 is an inducible enzyme, which is markedly overexpressed at sites of inflammation and colorectal neoplasms	topic_ccc
75143	2	355006	7	NULL	NULL	0	NULL	statement 1	Process		important role in					tissue homeostasis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	COX-1 is constitutively expressed in normal tissue, serving an important role in tissue homeostasis, whereas COX-2 is an inducible enzyme, which is markedly overexpressed at sites of inflammation and colorectal neoplasms	topic_ccc
75144	3	355006	7	NULL	NULL	0	NULL	COX-2	GP		is a type of					inducible enzyme	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	COX-1 is constitutively expressed in normal tissue, serving an important role in tissue homeostasis, whereas COX-2 is an inducible enzyme, which is markedly overexpressed at sites of inflammation and colorectal neoplasms	topic_ccc
75145	4	355006	7	NULL	NULL	0	NULL	COX-2	GP		overexpressed at		markedly			inflammation sites	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	COX-1 is constitutively expressed in normal tissue, serving an important role in tissue homeostasis, whereas COX-2 is an inducible enzyme, which is markedly overexpressed at sites of inflammation and colorectal neoplasms	topic_ccc
75146	5	355006	7	NULL	NULL	0	NULL	COX-2	GP		overexpressed at		markedly			colorectal neoplasms	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	COX-1 is constitutively expressed in normal tissue, serving an important role in tissue homeostasis, whereas COX-2 is an inducible enzyme, which is markedly overexpressed at sites of inflammation and colorectal neoplasms	topic_ccc
75147	1	355008	7	NULL	NULL	0	NULL	FOLFIRI plus BV	Chemical		treatment for					mCRC refractory 	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggest that FOLFIRI plus BV is a viable option in second-line treatment for mCRC refractory to first-line FOLFOX (5-fluorouracil, leucovorin, oxaliplatin) alone, and indicate that CA125 might be a predictive biomarker for the outcome.	topic_ccc
75148	1	355010	7	NULL	NULL	0	NULL	CRF	MedicalFinding		is a type of					 disabling symptom	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Cancer-related fatigue (CRF) is a disabling and distressing symptom that is highly prevalent across the cancer continuum from a patient's diagnosis and treatment through survivorship and end of life. 	topic_ccc
75149	2	355010	7	NULL	NULL	0	NULL	CRF	MedicalFinding		is a type of					distressing symptom 	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Cancer-related fatigue (CRF) is a disabling and distressing symptom that is highly prevalent across the cancer continuum from a patient's diagnosis and treatment through survivorship and end of life. 	topic_ccc
75150	3	355010	7	NULL	NULL	0	NULL	CRF	MedicalFinding		is					Cancer-related fatigue	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Cancer-related fatigue (CRF) is a disabling and distressing symptom that is highly prevalent across the cancer continuum from a patient's diagnosis and treatment through survivorship and end of life. 	topic_ccc
75151	1	355011	7	NULL	NULL	0	NULL	CC	MedicalFinding		 cancer in		common			women	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Cervical cancer (CC) is the third most common cancer in women worldwide; however, CC is a preventable disease, and much effort should be done to prevent it. Persistence of high-risk HPV infection is the strongest epidemiologic risk factor for CC, however it is not sufficient for development of the disease it cofactors should be present.	topic_ccc
75152	2	355011	7	NULL	NULL	0	NULL	CC	MedicalFinding		is a type of					preventable disease	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Cervical cancer (CC) is the third most common cancer in women worldwide; however, CC is a preventable disease, and much effort should be done to prevent it. Persistence of high-risk HPV infection is the strongest epidemiologic risk factor for CC, however it is not sufficient for development of the disease it cofactors should be present.	topic_ccc
75153	3	355011	7	NULL	NULL	0	NULL	HPV infection	MedicalFinding	Persistence of high-risk	epidemiologic risk factor		strongest			CC	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Cervical cancer (CC) is the third most common cancer in women worldwide; however, CC is a preventable disease, and much effort should be done to prevent it. Persistence of high-risk HPV infection is the strongest epidemiologic risk factor for CC, however it is not sufficient for development of the disease it cofactors should be present.	topic_ccc
75154	4	355011	7	NULL	NULL	0	NULL	CC	MedicalFinding		is					cervical cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Cervical cancer (CC) is the third most common cancer in women worldwide; however, CC is a preventable disease, and much effort should be done to prevent it. Persistence of high-risk HPV infection is the strongest epidemiologic risk factor for CC, however it is not sufficient for development of the disease it cofactors should be present.	topic_ccc
75155	1	355012	7	NULL	NULL	0	NULL	HPV	MedicalFinding		is a member of					Viruses	Organism	papillomavirus family of 			NULL		0	NULL	NULL	NULL	NULL	NULL	Human papillomavirus (HPV) is a member of the papillomavirus family of viruses that is capable of infecting humans.	topic_ccc
75156	2	355012	7	NULL	NULL	0	NULL	HPV	Organism		infect					humans	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Human papillomavirus (HPV) is a member of the papillomavirus family of viruses that is capable of infecting humans.	topic_ccc
75157	3	355012	7	NULL	NULL	0	NULL	HPV	Organism		is					Human papillomavirus	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Human papillomavirus (HPV) is a member of the papillomavirus family of viruses that is capable of infecting humans.	topic_ccc
75158	1	355013	7	NULL	NULL	0	NULL	abdominal obesity	MedicalFinding		is associated with					colon cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Among individual components, abdominal obesity (RR=1.51;95%CI:1.16-1.96) was associated with colon cancer	topic_ccc
75159	1	355014	7	NULL	NULL	0	NULL	HPV types 6	Organism		cause					genital warts	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	HPV types 6 and 11, which cause 90% of genital warts.	topic_ccc
75160	2	355014	7	NULL	NULL	0	NULL	HPV types 11	Organism		is a type of					genital warts	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	HPV types 6 and 11, which cause 90% of genital warts.	topic_ccc
75161	1	355015	7	NULL	NULL	0	NULL	HPV genome	Organism		is composed of					early E1 protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The HPV genome is composed of six early (E1, E2, E3, E4, E6, and E7) and two late (L1 and L2) proteins.	topic_ccc
75162	2	355015	7	NULL	NULL	0	NULL	HPV genome	Organism		is composed of					early E2 protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The HPV genome is composed of six early (E1, E2, E3, E4, E6, and E7) and two late (L1 and L2) proteins.	topic_ccc
75163	3	355015	7	NULL	NULL	NULL	NULL	HPV genome	Organism		is composed of					early E3 protein	GP				NULL		NULL	NULL	NULL	NULL	NULL	NULL	The HPV genome is composed of six early (E1, E2, E3, E4, E6, and E7) and two late (L1 and L2) proteins.	topic_ccc
75164	4	355015	7	NULL	NULL	0	NULL	HPV genome	Organism		is composed of					early E4 protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The HPV genome is composed of six early (E1, E2, E3, E4, E6, and E7) and two late (L1 and L2) proteins.	topic_ccc
75165	5	355015	7	NULL	NULL	0	NULL	HPV genome	Organism		is composed of					early E6 protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The HPV genome is composed of six early (E1, E2, E3, E4, E6, and E7) and two late (L1 and L2) proteins.	topic_ccc
75166	6	355015	7	NULL	NULL	0	NULL	HPV genome	Organism		is composed of					early E7 protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The HPV genome is composed of six early (E1, E2, E3, E4, E6, and E7) and two late (L1 and L2) proteins.	topic_ccc
75167	7	355015	7	NULL	NULL	0	NULL	HPV genome	Organism		is composed of					Late L1 protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The HPV genome is composed of six early (E1, E2, E3, E4, E6, and E7) and two late (L1 and L2) proteins.	topic_ccc
75168	8	355015	7	NULL	NULL	0	NULL	HPV genome	Organism		is composed of					Late L2 protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The HPV genome is composed of six early (E1, E2, E3, E4, E6, and E7) and two late (L1 and L2) proteins.	topic_ccc
75169	1	355016	7	NULL	NULL	0	NULL	E6 protein	GP		inactivates					p53	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	inactivation of tumor suppressor genes like p53 and pRB by HPV oncoproteins particularly E6 and E7	topic_ccc
75170	2	355016	7	NULL	NULL	0	NULL	E7 protein	GP		inactivates					pRB	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	inactivation of tumor suppressor genes like p53 and pRB by HPV oncoproteins particularly E6 and E7	topic_ccc
75171	3	355016	7	NULL	NULL	0	NULL	p53	GP		is a type of					tumor suppressor gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	inactivation of tumor suppressor genes like p53 and pRB by HPV oncoproteins particularly E6 and E7	topic_ccc
75172	4	355016	7	NULL	NULL	0	NULL	pRB	GP		is a type of					tumor suppressor gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	inactivation of tumor suppressor genes like p53 and pRB by HPV oncoproteins particularly E6 and E7	topic_ccc
75173	5	355016	7	NULL	NULL	NULL	NULL	E6 protein	GP		is a type of					HPV oncoprotein	GP				NULL		NULL	NULL	NULL	NULL	NULL	NULL	inactivation of tumor suppressor genes like p53 and pRB by HPV oncoproteins particularly E6 and E7	topic_ccc
75174	6	355016	7	NULL	NULL	0	NULL	E7 protein	GP		is a type of					HPV oncoprotein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	inactivation of tumor suppressor genes like p53 and pRB by HPV oncoproteins particularly E6 and E7	topic_ccc
75241	1	355018	7	NULL	NULL	0	NULL	HPV16 E6	GP		induce					p53	GP	ubiquitinated degradation of			NULL		0	NULL	NULL	NULL	NULL	NULL	The ubiquitinated degradation of p53 can be induced by human papillomavirus type 16 (HPV16) early gene 6 (E6); the phosphorylated inactivation of pRb can be induced by HPV16 E7.	topic_ccc
75242	2	355018	7	NULL	NULL	0	NULL	HPV16 E7	GP		induce					pRb	GP	phosphorylated inactivation of			NULL		0	NULL	NULL	NULL	NULL	NULL	The ubiquitinated degradation of p53 can be induced by human papillomavirus type 16 (HPV16) early gene 6 (E6); the phosphorylated inactivation of pRb can be induced by HPV16 E7.	topic_ccc
75243	3	355018	7	NULL	NULL	0	NULL	HPV16	Organism		is					human papillomavirus type 16	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	The ubiquitinated degradation of p53 can be induced by human papillomavirus type 16 (HPV16) early gene 6 (E6); the phosphorylated inactivation of pRb can be induced by HPV16 E7.	topic_ccc
75244	4	355018	7	NULL	NULL	0	NULL	E6	GP		is					early gene 6	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The ubiquitinated degradation of p53 can be induced by human papillomavirus type 16 (HPV16) early gene 6 (E6); the phosphorylated inactivation of pRb can be induced by HPV16 E7.	topic_ccc
75245	1	355019	7	NULL	NULL	NULL	NULL	E6	GP		is involved in					beta-catenin	GP	nuclear accumulation of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Thus, E6 and E7 are involved in beta-catenin nuclear accumulation and activation of Wnt signaling in HPV-induced cancers.	topic_ccc
75246	2	355019	7	NULL	NULL	0	NULL	E7	GP		is involved in					beta-catenin	GP	nuclear accumulation of			NULL		0	NULL	NULL	NULL	NULL	NULL	Thus, E6 and E7 are involved in beta-catenin nuclear accumulation and activation of Wnt signaling in HPV-induced cancers.	topic_ccc
75247	3	355019	7	NULL	NULL	NULL	NULL	E6	GP		is involved in					Wnt signaling	Process	activation of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Thus, E6 and E7 are involved in beta-catenin nuclear accumulation and activation of Wnt signaling in HPV-induced cancers.	topic_ccc
75248	4	355019	7	NULL	NULL	NULL	NULL	E7	GP		is involved in					Wnt signaling	Process	activation of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Thus, E6 and E7 are involved in beta-catenin nuclear accumulation and activation of Wnt signaling in HPV-induced cancers.	topic_ccc
75249	5	355019	7	NULL	NULL	0	NULL	statement 1	Process		occur in					HPV-induced cancers	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Thus, E6 and E7 are involved in beta-catenin nuclear accumulation and activation of Wnt signaling in HPV-induced cancers.	topic_ccc
75250	6	355019	7	NULL	NULL	NULL	NULL	statement 2	Process		occur in					HPV-induced cancers	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Thus, E6 and E7 are involved in beta-catenin nuclear accumulation and activation of Wnt signaling in HPV-induced cancers.	topic_ccc
75251	7	355019	7	NULL	NULL	0	NULL	statement 3	Process		occur in					HPV-induced cancers	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Thus, E6 and E7 are involved in beta-catenin nuclear accumulation and activation of Wnt signaling in HPV-induced cancers.	topic_ccc
75252	8	355019	7	NULL	NULL	0	NULL	statement 4	Process		occur in					HPV-induced cancers	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Thus, E6 and E7 are involved in beta-catenin nuclear accumulation and activation of Wnt signaling in HPV-induced cancers.	topic_ccc
75253	1	355020	7	NULL	NULL	0	NULL	HPV16 E6	GP		induce					p53	GP	ubiquitinated degradation of			NULL		0	NULL	NULL	NULL	NULL	NULL	The ubiquitinated degradation of p53 can be induced by human papillomavirus type 16 (HPV16) early gene 6 (E6); the phosphorylated inactivation of pRb can be induced by HPV16 E7. They are closely associated with the carcinogenesis and progression of cervical cancer.	topic_ccc
75254	2	355020	7	NULL	NULL	0	NULL	HPV16 E7	GP		induce					pRb	GP	phosphorylated inactivation of			NULL		0	NULL	NULL	NULL	NULL	NULL	The ubiquitinated degradation of p53 can be induced by human papillomavirus type 16 (HPV16) early gene 6 (E6); the phosphorylated inactivation of pRb can be induced by HPV16 E7. They are closely associated with the carcinogenesis and progression of cervical cancer.	topic_ccc
75255	3	355020	7	NULL	NULL	0	NULL	HPV16 	Organism		is					human papillomavirus type 16	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	The ubiquitinated degradation of p53 can be induced by human papillomavirus type 16 (HPV16) early gene 6 (E6); the phosphorylated inactivation of pRb can be induced by HPV16 E7. They are closely associated with the carcinogenesis and progression of cervical cancer.	topic_ccc
75256	4	355020	7	NULL	NULL	0	NULL	E6	GP		is 					early gene 6	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The ubiquitinated degradation of p53 can be induced by human papillomavirus type 16 (HPV16) early gene 6 (E6); the phosphorylated inactivation of pRb can be induced by HPV16 E7. They are closely associated with the carcinogenesis and progression of cervical cancer.	topic_ccc
75257	5	355020	7	NULL	NULL	NULL	NULL	statement 1	Process		associated with		closely			cervical cancer	MedicalFinding	carcinogenesis of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ubiquitinated degradation of p53 can be induced by human papillomavirus type 16 (HPV16) early gene 6 (E6); the phosphorylated inactivation of pRb can be induced by HPV16 E7. They are closely associated with the carcinogenesis and progression of cervical cancer.	topic_ccc
75258	6	355020	7	NULL	NULL	0	NULL	statement 1	Process		is associated with		closely			cervical cancer	MedicalFinding	progression of			NULL		0	NULL	NULL	NULL	NULL	NULL	The ubiquitinated degradation of p53 can be induced by human papillomavirus type 16 (HPV16) early gene 6 (E6); the phosphorylated inactivation of pRb can be induced by HPV16 E7. They are closely associated with the carcinogenesis and progression of cervical cancer.	topic_ccc
75259	7	355020	7	NULL	NULL	0	NULL	statement 5	Process		occur simultaneously with					statement 6	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The ubiquitinated degradation of p53 can be induced by human papillomavirus type 16 (HPV16) early gene 6 (E6); the phosphorylated inactivation of pRb can be induced by HPV16 E7. They are closely associated with the carcinogenesis and progression of cervical cancer.	topic_ccc
75260	8	355020	7	NULL	NULL	0	NULL	statement 2	Process		associated with		closely			cervical cancer	MedicalFinding	carcinogenesis of			NULL		0	NULL	NULL	NULL	NULL	NULL	The ubiquitinated degradation of p53 can be induced by human papillomavirus type 16 (HPV16) early gene 6 (E6); the phosphorylated inactivation of pRb can be induced by HPV16 E7. They are closely associated with the carcinogenesis and progression of cervical cancer.	topic_ccc
75261	9	355020	7	NULL	NULL	0	NULL	statement 2	Process		associated with		closely			cervical cancer	MedicalFinding	progression of			NULL		0	NULL	NULL	NULL	NULL	NULL	The ubiquitinated degradation of p53 can be induced by human papillomavirus type 16 (HPV16) early gene 6 (E6); the phosphorylated inactivation of pRb can be induced by HPV16 E7. They are closely associated with the carcinogenesis and progression of cervical cancer.	topic_ccc
75262	10	355020	7	NULL	NULL	0	NULL	statement 8	Process		occur simultaneously with					statement 9	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The ubiquitinated degradation of p53 can be induced by human papillomavirus type 16 (HPV16) early gene 6 (E6); the phosphorylated inactivation of pRb can be induced by HPV16 E7. They are closely associated with the carcinogenesis and progression of cervical cancer.	topic_ccc
75263	1	355022	7	NULL	NULL	0	NULL	E2F	GP	transcription activities of	suppressed by					peptide	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Luciferase reporter assay verified that transcription activities of E2F were suppressed by the peptide through restoration of pRb.	topic_ccc
75264	2	355022	7	NULL	NULL	0	NULL	statement 1	Process		occur through					pRb	GP	restoration of			NULL		0	NULL	NULL	NULL	NULL	NULL	Luciferase reporter assay verified that transcription activities of E2F were suppressed by the peptide through restoration of pRb.	topic_ccc
75265	1	355024	7	NULL	NULL	NULL	NULL	HPV	Organism	High-risk;;oncogenic type	cause					cervical cancer	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	High-risk or oncogenic types of HPV cause cervical, vaginal, and vulvar cancer in women.	topic_ccc
75266	2	355024	7	NULL	NULL	0	NULL	HPV	Organism	High-risk;;oncogenic type	cause					vaginal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	High-risk or oncogenic types of HPV cause cervical, vaginal, and vulvar cancer in women.	topic_ccc
75267	3	355024	7	NULL	NULL	0	NULL	HPV	Organism	High-risk;;oncogenic type	cause					vulvar cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	High-risk or oncogenic types of HPV cause cervical, vaginal, and vulvar cancer in women.	topic_ccc
75268	4	355024	7	NULL	NULL	0	NULL	statement 1	Process		occur in					women	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	High-risk or oncogenic types of HPV cause cervical, vaginal, and vulvar cancer in women.	topic_ccc
75269	5	355024	7	NULL	NULL	0	NULL	statement 2	Process		occur in					women	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	High-risk or oncogenic types of HPV cause cervical, vaginal, and vulvar cancer in women.	topic_ccc
75270	6	355024	7	NULL	NULL	0	NULL	statement 3	Process		occur in					women	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	High-risk or oncogenic types of HPV cause cervical, vaginal, and vulvar cancer in women.	topic_ccc
75271	1	355025	7	NULL	NULL	0	NULL	primary oropharyngeal cancers	MedicalFinding		is related to					HR-HPV	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	The association between squamous cell carcinoma of the head and neck (HNSCC) and infection with human papilloma viruses (HPV) has created considerable interest. Rates of primary oropharyngeal cancers have shown increasing incidence and declining age at presentation over the last decade, believed to relate to infection with oncogenic or high-risk subtypes of HPV (HR-HPV).	topic_ccc
75272	2	355025	7	NULL	NULL	NULL	NULL	HR-HPV	Organism		is 					high-risk HPV	Organism				NULL		NULL	NULL	NULL	NULL	NULL	NULL	The association between squamous cell carcinoma of the head and neck (HNSCC) and infection with human papilloma viruses (HPV) has created considerable interest. Rates of primary oropharyngeal cancers have shown increasing incidence and declining age at presentation over the last decade, believed to relate to infection with oncogenic or high-risk subtypes of HPV (HR-HPV).	topic_ccc
75273	3	355025	7	NULL	NULL	0	NULL	HR-HPV	Organism		is					oncogenic HPV	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	The association between squamous cell carcinoma of the head and neck (HNSCC) and infection with human papilloma viruses (HPV) has created considerable interest. Rates of primary oropharyngeal cancers have shown increasing incidence and declining age at presentation over the last decade, believed to relate to infection with oncogenic or high-risk subtypes of HPV (HR-HPV).	topic_ccc
75274	4	355025	7	NULL	NULL	0	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The association between squamous cell carcinoma of the head and neck (HNSCC) and infection with human papilloma viruses (HPV) has created considerable interest. Rates of primary oropharyngeal cancers have shown increasing incidence and declining age at presentation over the last decade, believed to relate to infection with oncogenic or high-risk subtypes of HPV (HR-HPV).	topic_ccc
75275	1	355026	7	NULL	NULL	0	NULL	Aberrant DNA methylation	Process		molecular features of					CRCs	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Aberrant DNA methylation, Microsatellite Instability (MSI) and Chromosomal Instability (CIN) are well-characterised molecular features of sporadic colorectal cancers (CRCs). In addition to CpG island methylator phenotype (CIMP) associated with MSI, an intermediate methylation subgroup is also a feature of non-MSI cancers.	topic_ccc
75276	2	355026	7	NULL	NULL	0	NULL	MSI	Process		molecular features of					CRCs	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Aberrant DNA methylation, Microsatellite Instability (MSI) and Chromosomal Instability (CIN) are well-characterised molecular features of sporadic colorectal cancers (CRCs). In addition to CpG island methylator phenotype (CIMP) associated with MSI, an intermediate methylation subgroup is also a feature of non-MSI cancers.	topic_ccc
75277	3	355026	7	NULL	NULL	0	NULL	CIN	Process		molecular features of					CRCs	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Aberrant DNA methylation, Microsatellite Instability (MSI) and Chromosomal Instability (CIN) are well-characterised molecular features of sporadic colorectal cancers (CRCs). In addition to CpG island methylator phenotype (CIMP) associated with MSI, an intermediate methylation subgroup is also a feature of non-MSI cancers.	topic_ccc
75278	4	355026	7	NULL	NULL	0	NULL	CIMP	PhysicalPhenomenon		associated with					MSI	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Aberrant DNA methylation, Microsatellite Instability (MSI) and Chromosomal Instability (CIN) are well-characterised molecular features of sporadic colorectal cancers (CRCs). In addition to CpG island methylator phenotype (CIMP) associated with MSI, an intermediate methylation subgroup is also a feature of non-MSI cancers.	topic_ccc
75279	6	355026	7	NULL	NULL	NULL	NULL	statement 4	Process		feature of					non-MSI cancer	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Aberrant DNA methylation, Microsatellite Instability (MSI) and Chromosomal Instability (CIN) are well-characterised molecular features of sporadic colorectal cancers (CRCs). In addition to CpG island methylator phenotype (CIMP) associated with MSI, an intermediate methylation subgroup is also a feature of non-MSI cancers.	topic_ccc
75280	7	355026	7	NULL	NULL	NULL	NULL	 intermediate methylation subgroup	Chemical		is a feature of					non-MSI cancer	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Aberrant DNA methylation, Microsatellite Instability (MSI) and Chromosomal Instability (CIN) are well-characterised molecular features of sporadic colorectal cancers (CRCs). In addition to CpG island methylator phenotype (CIMP) associated with MSI, an intermediate methylation subgroup is also a feature of non-MSI cancers.	topic_ccc
75281	8	355026	7	NULL	NULL	0	NULL	MSI	Process		is					Microsatellite Instability	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Aberrant DNA methylation, Microsatellite Instability (MSI) and Chromosomal Instability (CIN) are well-characterised molecular features of sporadic colorectal cancers (CRCs). In addition to CpG island methylator phenotype (CIMP) associated with MSI, an intermediate methylation subgroup is also a feature of non-MSI cancers.	topic_ccc
75282	9	355026	7	NULL	NULL	0	NULL	CIN	Process		is					Chromosomal Instability	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Aberrant DNA methylation, Microsatellite Instability (MSI) and Chromosomal Instability (CIN) are well-characterised molecular features of sporadic colorectal cancers (CRCs). In addition to CpG island methylator phenotype (CIMP) associated with MSI, an intermediate methylation subgroup is also a feature of non-MSI cancers.	topic_ccc
75283	10	355026	7	NULL	NULL	0	NULL	CRCs	MedicalFinding		is					sporadic colorectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Aberrant DNA methylation, Microsatellite Instability (MSI) and Chromosomal Instability (CIN) are well-characterised molecular features of sporadic colorectal cancers (CRCs). In addition to CpG island methylator phenotype (CIMP) associated with MSI, an intermediate methylation subgroup is also a feature of non-MSI cancers.	topic_ccc
75284	11	355026	7	NULL	NULL	0	NULL	CIMP	PhysicalPhenomenon		is					CpG island methylator phenotype	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	NULL	NULL	Aberrant DNA methylation, Microsatellite Instability (MSI) and Chromosomal Instability (CIN) are well-characterised molecular features of sporadic colorectal cancers (CRCs). In addition to CpG island methylator phenotype (CIMP) associated with MSI, an intermediate methylation subgroup is also a feature of non-MSI cancers.	topic_ccc
75287	1	355027	7	NULL	NULL	0	NULL	hMLH1	GP		shows					tubular adenomas	MedicalFinding	specific methylation profiles for			NULL		0	NULL	NULL	NULL	NULL	NULL	Methylation analysis of hMLH1, CDKN2A/p16, and MGMT revealed specific methylation profiles for tubular adenomas, tubulovillous/villous adenomas, and colorectal cancers, supporting the use of these alterations in assessment of colorectal tumorigenesis.	topic_ccc
75288	2	355027	7	NULL	NULL	NULL	NULL	CDKN2A/p16	GP		shows					tubular adenomas	MedicalFinding	specific methylation profiles for			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Methylation analysis of hMLH1, CDKN2A/p16, and MGMT revealed specific methylation profiles for tubular adenomas, tubulovillous/villous adenomas, and colorectal cancers, supporting the use of these alterations in assessment of colorectal tumorigenesis.	topic_ccc
75291	3	355027	7	NULL	NULL	0	NULL	MGMT	GP		shows					tubular adenomas	MedicalFinding	specific methylation profiles for			NULL		0	NULL	NULL	NULL	NULL	NULL	Methylation analysis of hMLH1, CDKN2A/p16, and MGMT revealed specific methylation profiles for tubular adenomas, tubulovillous/villous adenomas, and colorectal cancers, supporting the use of these alterations in assessment of colorectal tumorigenesis.	topic_ccc
75292	4	355027	7	NULL	NULL	0	NULL	hMLH1	GP		shows					tubulovillous/villous adenomas	MedicalFinding	specific methylation profiles for			NULL		0	NULL	NULL	NULL	NULL	NULL	Methylation analysis of hMLH1, CDKN2A/p16, and MGMT revealed specific methylation profiles for tubular adenomas, tubulovillous/villous adenomas, and colorectal cancers, supporting the use of these alterations in assessment of colorectal tumorigenesis.	topic_ccc
75293	5	355027	7	NULL	NULL	0	NULL	CDKN2A/p16	GP		shows					tubulovillous/villous adenomas	MedicalFinding	specific methylation profiles for			NULL		0	NULL	NULL	NULL	NULL	NULL	Methylation analysis of hMLH1, CDKN2A/p16, and MGMT revealed specific methylation profiles for tubular adenomas, tubulovillous/villous adenomas, and colorectal cancers, supporting the use of these alterations in assessment of colorectal tumorigenesis.	topic_ccc
75295	6	355027	7	NULL	NULL	0	NULL	MGMT	GP		shows					tubulovillous/villous adenomas	MedicalFinding	specific methylation profiles for			NULL		0	NULL	NULL	NULL	NULL	NULL	Methylation analysis of hMLH1, CDKN2A/p16, and MGMT revealed specific methylation profiles for tubular adenomas, tubulovillous/villous adenomas, and colorectal cancers, supporting the use of these alterations in assessment of colorectal tumorigenesis.	topic_ccc
75299	7	355027	7	NULL	NULL	NULL	NULL	hMLH1	GP		shows					colorectal cancers	MedicalFinding	specific methylation profiles for			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Methylation analysis of hMLH1, CDKN2A/p16, and MGMT revealed specific methylation profiles for tubular adenomas, tubulovillous/villous adenomas, and colorectal cancers, supporting the use of these alterations in assessment of colorectal tumorigenesis.	topic_ccc
75300	8	355027	7	NULL	NULL	0	NULL	CDKN2A/p16	GP		shows					colorectal cancers	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Methylation analysis of hMLH1, CDKN2A/p16, and MGMT revealed specific methylation profiles for tubular adenomas, tubulovillous/villous adenomas, and colorectal cancers, supporting the use of these alterations in assessment of colorectal tumorigenesis.	topic_ccc
75301	9	355027	7	NULL	NULL	0	NULL	MGMT	GP		shows					colorectal cancers	MedicalFinding	specific methylation profiles for			NULL		0	NULL	NULL	NULL	NULL	NULL	Methylation analysis of hMLH1, CDKN2A/p16, and MGMT revealed specific methylation profiles for tubular adenomas, tubulovillous/villous adenomas, and colorectal cancers, supporting the use of these alterations in assessment of colorectal tumorigenesis.	topic_ccc
75317	1	355029	7	NULL	NULL	NULL	NULL	DNA methylation 	Process	anomalies in	include					CIMP1	PhysicalPhenomenon				NULL		NULL	NULL	NULL	NULL	NULL	NULL	In colorectal cancer (CRC), DNA methylation anomalies define distinct subgroups termed CpG island methylator phenotype 1 (CIMP1), CIMP2, and CIMP-negative.	topic_ccc
75318	2	355029	7	NULL	NULL	NULL	NULL	DNA methylation 	Process	anomalies in	include					CIMP2	PhysicalPhenomenon				NULL		NULL	NULL	NULL	NULL	NULL	NULL	In colorectal cancer (CRC), DNA methylation anomalies define distinct subgroups termed CpG island methylator phenotype 1 (CIMP1), CIMP2, and CIMP-negative.	topic_ccc
75319	3	355029	7	NULL	NULL	NULL	NULL	DNA methylation 	Process	anomalies in	include					CIMP-negative	PhysicalPhenomenon				NULL		NULL	NULL	NULL	NULL	NULL	NULL	In colorectal cancer (CRC), DNA methylation anomalies define distinct subgroups termed CpG island methylator phenotype 1 (CIMP1), CIMP2, and CIMP-negative.	topic_ccc
75320	4	355029	7	NULL	NULL	0	NULL	statement 1	Process		occur in					CRC	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In colorectal cancer (CRC), DNA methylation anomalies define distinct subgroups termed CpG island methylator phenotype 1 (CIMP1), CIMP2, and CIMP-negative.	topic_ccc
75321	5	355029	7	NULL	NULL	0	NULL	statement 2	Process		occur in					CRC	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In colorectal cancer (CRC), DNA methylation anomalies define distinct subgroups termed CpG island methylator phenotype 1 (CIMP1), CIMP2, and CIMP-negative.	topic_ccc
75322	6	355029	7	NULL	NULL	0	NULL	statement 3	Process		occur in					CRC	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In colorectal cancer (CRC), DNA methylation anomalies define distinct subgroups termed CpG island methylator phenotype 1 (CIMP1), CIMP2, and CIMP-negative.	topic_ccc
75323	7	355029	7	NULL	NULL	0	NULL	CRC	MedicalFinding		is					colorectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In colorectal cancer (CRC), DNA methylation anomalies define distinct subgroups termed CpG island methylator phenotype 1 (CIMP1), CIMP2, and CIMP-negative.	topic_ccc
75324	8	355029	7	NULL	NULL	0	NULL	CIMP1	PhysicalPhenomenon		is					CpG island methylator phenotype 1	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	NULL	NULL	In colorectal cancer (CRC), DNA methylation anomalies define distinct subgroups termed CpG island methylator phenotype 1 (CIMP1), CIMP2, and CIMP-negative.	topic_ccc
75325	1	355030	7	NULL	NULL	NULL	NULL	AMPK	GP	activation of	suppress		strongly			cell proliferation	Process				NULL	nonmalignant cells	NULL	NULL	NULL	NULL	NULL	NULL	Activation of AMP-activated protein kinase (AMPK), a physiological cellular energy sensor, strongly suppresses cell proliferation in both nonmalignant and tumor cells. 	topic_ccc
75326	2	355030	7	NULL	NULL	NULL	NULL	AMPK	GP	activation of	suppress		strongly			cell proliferation	Process				NULL	tumor cells	NULL	NULL	NULL	NULL	NULL	NULL	Activation of AMP-activated protein kinase (AMPK), a physiological cellular energy sensor, strongly suppresses cell proliferation in both nonmalignant and tumor cells. 	topic_ccc
75327	3	355030	7	NULL	NULL	0	NULL	AMPK	GP		is					AMP-activated protein kinase	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of AMP-activated protein kinase (AMPK), a physiological cellular energy sensor, strongly suppresses cell proliferation in both nonmalignant and tumor cells. 	topic_ccc
75328	4	355030	7	NULL	NULL	0	NULL	AMPK	GP		is a type of					physiological cellular energy sensor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of AMP-activated protein kinase (AMPK), a physiological cellular energy sensor, strongly suppresses cell proliferation in both nonmalignant and tumor cells. 	topic_ccc
75329	1	355032	7	NULL	NULL	0	NULL	ras p21 Oncoprotein	GP	expression of	is related to					K-ras Gene	GP	mutation status of			NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship Between Expression of ras p21 Oncoprotein and Mutation Status of the K-ras Gene in Sporadic Colorectal Cancer Patients in Tunisia.	topic_ccc
75330	2	355032	7	NULL	NULL	0	NULL	statement 1	Process		occur in					Sporadic Colorectal Cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship Between Expression of ras p21 Oncoprotein and Mutation Status of the K-ras Gene in Sporadic Colorectal Cancer Patients in Tunisia.	topic_ccc
75331	1	355033	7	NULL	NULL	0	NULL	quercetin 	Chemical		induce					apoptosis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	All of these results indicate that quercetin induces apoptosis via AMPK activation and p53-dependent apoptotic cell death in HT-29 colon cancer cells and that it may be a potential chemopreventive or therapeutic agent against HT-29 colon cancer.	topic_ccc
75332	2	355033	7	NULL	NULL	0	NULL	statement 1	Process		via					AMPK	GP	activation of			NULL		0	NULL	NULL	NULL	NULL	NULL	All of these results indicate that quercetin induces apoptosis via AMPK activation and p53-dependent apoptotic cell death in HT-29 colon cancer cells and that it may be a potential chemopreventive or therapeutic agent against HT-29 colon cancer.	topic_ccc
75333	3	355033	7	NULL	NULL	0	NULL	apoptotic cell death	Process		depends on					p53	GP				NULL	HT-29 colon cancer cells	0	NULL	NULL	NULL	NULL	NULL	All of these results indicate that quercetin induces apoptosis via AMPK activation and p53-dependent apoptotic cell death in HT-29 colon cancer cells and that it may be a potential chemopreventive or therapeutic agent against HT-29 colon cancer.	topic_ccc
75334	4	355033	7	NULL	NULL	0	NULL	statement 1	Process		via					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	All of these results indicate that quercetin induces apoptosis via AMPK activation and p53-dependent apoptotic cell death in HT-29 colon cancer cells and that it may be a potential chemopreventive or therapeutic agent against HT-29 colon cancer.	topic_ccc
75335	5	355033	7	NULL	NULL	0	NULL	statement 2	Process		occur along with					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	All of these results indicate that quercetin induces apoptosis via AMPK activation and p53-dependent apoptotic cell death in HT-29 colon cancer cells and that it may be a potential chemopreventive or therapeutic agent against HT-29 colon cancer.	topic_ccc
75336	6	355033	7	NULL	NULL	NULL	NULL	quercetin 	Chemical		chemopreventive agent against		potential			HT-29 colon cancer	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	All of these results indicate that quercetin induces apoptosis via AMPK activation and p53-dependent apoptotic cell death in HT-29 colon cancer cells and that it may be a potential chemopreventive or therapeutic agent against HT-29 colon cancer.	topic_ccc
75337	7	355033	7	NULL	NULL	NULL	NULL	quercetin 	Chemical		therapeutic agent against		potential			HT-29 colon cancer	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	All of these results indicate that quercetin induces apoptosis via AMPK activation and p53-dependent apoptotic cell death in HT-29 colon cancer cells and that it may be a potential chemopreventive or therapeutic agent against HT-29 colon cancer.	topic_ccc
75338	8	355033	7	NULL	NULL	0	NULL	statement 6	Process		is an alternative to					statement 7	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	All of these results indicate that quercetin induces apoptosis via AMPK activation and p53-dependent apoptotic cell death in HT-29 colon cancer cells and that it may be a potential chemopreventive or therapeutic agent against HT-29 colon cancer.	topic_ccc
75339	1	355034	7	NULL	NULL	NULL	NULL	silibinin	Chemical	antitumor efficacy of	against					CRC	MedicalFinding				NULL	in vivo	NULL	NULL	NULL	NULL	NULL	NULL	These findings suggest in vivo antitumor efficacy of silibinin against CRC involving its antiproliferative, proapoptotic, and antiangiogenic activities.	topic_ccc
75340	2	355034	7	NULL	NULL	0	NULL	statement 1	Process		involves					antiproliferative activities	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest in vivo antitumor efficacy of silibinin against CRC involving its antiproliferative, proapoptotic, and antiangiogenic activities.	topic_ccc
75341	3	355034	7	NULL	NULL	0	NULL	statement 1	Process		involves					proapoptotic activities	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest in vivo antitumor efficacy of silibinin against CRC involving its antiproliferative, proapoptotic, and antiangiogenic activities.	topic_ccc
75342	4	355034	7	NULL	NULL	0	NULL	statement 1	Process		involves					antiangiogenic activities	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest in vivo antitumor efficacy of silibinin against CRC involving its antiproliferative, proapoptotic, and antiangiogenic activities.	topic_ccc
75343	1	355035	7	NULL	NULL	NULL	NULL	silibinin	Chemical		inhibits					cell proliferation	Process				NULL	tissue samples	NULL	NULL	NULL	NULL	NULL	NULL	Mechanistic studies in tissue samples showed that silibinin inhibits cell proliferation as evident by a decrease (P < 0.001) in proliferating cell nuclear antigen and cyclin D1, and increased Cip1/p21 levels.	topic_ccc
75344	2	355035	7	NULL	NULL	NULL	NULL	silibinin	Chemical		decrease					proliferating cell nuclear antigen	GP	levels of			NULL	tissue samples	NULL	NULL	NULL	NULL	NULL	NULL	Mechanistic studies in tissue samples showed that silibinin inhibits cell proliferation as evident by a decrease (P < 0.001) in proliferating cell nuclear antigen and cyclin D1, and increased Cip1/p21 levels.	topic_ccc
75345	3	355035	7	NULL	NULL	NULL	NULL	silibinin	Chemical		decrease					cyclin D1	GP	levels of			NULL	tissue samples	NULL	NULL	NULL	NULL	NULL	NULL	Mechanistic studies in tissue samples showed that silibinin inhibits cell proliferation as evident by a decrease (P < 0.001) in proliferating cell nuclear antigen and cyclin D1, and increased Cip1/p21 levels.	topic_ccc
75346	4	355035	7	NULL	NULL	NULL	NULL	silibinin	Chemical		increase					Cip1/p21	GP	levels of			NULL	tissue samples	NULL	NULL	NULL	NULL	NULL	NULL	Mechanistic studies in tissue samples showed that silibinin inhibits cell proliferation as evident by a decrease (P < 0.001) in proliferating cell nuclear antigen and cyclin D1, and increased Cip1/p21 levels.	topic_ccc
75347	1	355036	7	NULL	NULL	NULL	NULL	 silibinin	Chemical		chemopreventive agent against					CRC HT29 xenograft growth	MedicalFinding	human			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Herein, for the first time, we investigated in vivo efficacy and associated molecular biomarkers and mechanisms of a chemopreventive agent, silibinin, against human colorectal carcinoma (CRC) HT29 xenograft growth.	topic_ccc
75348	2	355036	7	NULL	NULL	0	NULL	CRC	MedicalFinding		is					colorectal carcinoma 	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Herein, for the first time, we investigated in vivo efficacy and associated molecular biomarkers and mechanisms of a chemopreventive agent, silibinin, against human colorectal carcinoma (CRC) HT29 xenograft growth.	topic_ccc
75349	1	355037	7	NULL	NULL	0	NULL	silibinin	Chemical	Antiangiogenic effect of 	coupled with					inducible NOS	GP	strong decrease in			NULL		0	NULL	NULL	NULL	NULL	NULL	 Antiangiogenic effect of silibinin was coupled with a strong decrease in inducible nitric oxide synthase (NOS) and NOS3, cyclooxygenase-1 (COX-1) and COX-2, and hypoxia-inducing factor-1 alpha (HIF-1 alpha) and vascular endothelial growth factor (VEGF).	topic_ccc
75350	2	355037	7	NULL	NULL	0	NULL	silibinin	Chemical	Antiangiogenic effect of 	coupled with					NOS3	GP	strong decrease in			NULL		0	NULL	NULL	NULL	NULL	NULL	 Antiangiogenic effect of silibinin was coupled with a strong decrease in inducible nitric oxide synthase (NOS) and NOS3, cyclooxygenase-1 (COX-1) and COX-2, and hypoxia-inducing factor-1 alpha (HIF-1 alpha) and vascular endothelial growth factor (VEGF).	topic_ccc
75351	3	355037	7	NULL	NULL	0	NULL	silibinin	Chemical	Antiangiogenic effect of 	coupled with					COX-1	GP	strong decrease in			NULL		0	NULL	NULL	NULL	NULL	NULL	 Antiangiogenic effect of silibinin was coupled with a strong decrease in inducible nitric oxide synthase (NOS) and NOS3, cyclooxygenase-1 (COX-1) and COX-2, and hypoxia-inducing factor-1 alpha (HIF-1 alpha) and vascular endothelial growth factor (VEGF).	topic_ccc
75352	4	355037	7	NULL	NULL	0	NULL	silibinin	Chemical	Antiangiogenic effect of 	coupled with					COX-2	GP	strong decrease in			NULL		0	NULL	NULL	NULL	NULL	NULL	 Antiangiogenic effect of silibinin was coupled with a strong decrease in inducible nitric oxide synthase (NOS) and NOS3, cyclooxygenase-1 (COX-1) and COX-2, and hypoxia-inducing factor-1 alpha (HIF-1 alpha) and vascular endothelial growth factor (VEGF).	topic_ccc
75353	5	355037	7	NULL	NULL	NULL	NULL	silibinin	Chemical	Antiangiogenic effect of 	coupled with					HIF-1 alpha	GP	strong decrease in			NULL		NULL	NULL	NULL	NULL	NULL	NULL	 Antiangiogenic effect of silibinin was coupled with a strong decrease in inducible nitric oxide synthase (NOS) and NOS3, cyclooxygenase-1 (COX-1) and COX-2, and hypoxia-inducing factor-1 alpha (HIF-1 alpha) and vascular endothelial growth factor (VEGF).	topic_ccc
75354	6	355037	7	NULL	NULL	0	NULL	silibinin	Chemical	Antiangiogenic effect of 	coupled with					VEGF	GP	strong decrease in			NULL		0	NULL	NULL	NULL	NULL	NULL	 Antiangiogenic effect of silibinin was coupled with a strong decrease in inducible nitric oxide synthase (NOS) and NOS3, cyclooxygenase-1 (COX-1) and COX-2, and hypoxia-inducing factor-1 alpha (HIF-1 alpha) and vascular endothelial growth factor (VEGF).	topic_ccc
75355	7	355037	7	NULL	NULL	0	NULL	NOS	GP		is					nitric oxide synthase	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 Antiangiogenic effect of silibinin was coupled with a strong decrease in inducible nitric oxide synthase (NOS) and NOS3, cyclooxygenase-1 (COX-1) and COX-2, and hypoxia-inducing factor-1 alpha (HIF-1 alpha) and vascular endothelial growth factor (VEGF).	topic_ccc
75356	8	355037	7	NULL	NULL	0	NULL	COX-1	GP		is					cyclooxygenase-1	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 Antiangiogenic effect of silibinin was coupled with a strong decrease in inducible nitric oxide synthase (NOS) and NOS3, cyclooxygenase-1 (COX-1) and COX-2, and hypoxia-inducing factor-1 alpha (HIF-1 alpha) and vascular endothelial growth factor (VEGF).	topic_ccc
75357	9	355037	7	NULL	NULL	0	NULL	HIF-1 alpha	GP		is					hypoxia-inducing factor-1 alpha	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 Antiangiogenic effect of silibinin was coupled with a strong decrease in inducible nitric oxide synthase (NOS) and NOS3, cyclooxygenase-1 (COX-1) and COX-2, and hypoxia-inducing factor-1 alpha (HIF-1 alpha) and vascular endothelial growth factor (VEGF).	topic_ccc
75358	10	355037	7	NULL	NULL	0	NULL	VEGF	GP		is					vascular endothelial growth factor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 Antiangiogenic effect of silibinin was coupled with a strong decrease in inducible nitric oxide synthase (NOS) and NOS3, cyclooxygenase-1 (COX-1) and COX-2, and hypoxia-inducing factor-1 alpha (HIF-1 alpha) and vascular endothelial growth factor (VEGF).	topic_ccc
75359	1	355038	7	NULL	NULL	0	NULL	Pak1	GP		overexpressed in					colorectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Pak1 has been reported to be overexpressed in colorectal cancer, but the role of Pak1 in colorectal cancer remains unclear.	topic_ccc
75360	1	355039	7	NULL	NULL	0	NULL	Pak1	GP	overexpression of	increase					cell motility	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 Overexpression of Pak1 increased colorectal cancer cell motility and invasion, whereas down-regulation of Pak1 expression or activity reduced colorectal cancer cell migration and invasion.	topic_ccc
75361	2	355039	7	NULL	NULL	0	NULL	Pak1	GP	overexpression of	increase					cell invasion	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 Overexpression of Pak1 increased colorectal cancer cell motility and invasion, whereas down-regulation of Pak1 expression or activity reduced colorectal cancer cell migration and invasion.	topic_ccc
75362	3	355039	7	NULL	NULL	0	NULL	statement 1	Process		occur in					colorectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	 Overexpression of Pak1 increased colorectal cancer cell motility and invasion, whereas down-regulation of Pak1 expression or activity reduced colorectal cancer cell migration and invasion.	topic_ccc
75363	4	355039	7	NULL	NULL	0	NULL	statement 2	Process		occur in					colorectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	 Overexpression of Pak1 increased colorectal cancer cell motility and invasion, whereas down-regulation of Pak1 expression or activity reduced colorectal cancer cell migration and invasion.	topic_ccc
75364	5	355039	7	NULL	NULL	0	NULL	Pak1	GP	down-regulation of ;;expression of	reduce					colorectal cancer cell migration 	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 Overexpression of Pak1 increased colorectal cancer cell motility and invasion, whereas down-regulation of Pak1 expression or activity reduced colorectal cancer cell migration and invasion.	topic_ccc
75365	6	355039	7	NULL	NULL	0	NULL	Pak1	GP	down-regulation of ;;expression of	reduce					colorectal cell invasion	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 Overexpression of Pak1 increased colorectal cancer cell motility and invasion, whereas down-regulation of Pak1 expression or activity reduced colorectal cancer cell migration and invasion.	topic_ccc
75366	1	355040	7	NULL	NULL	0	NULL	Chk1	GP	initial	involved in					G(2) arrest	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 We revealed subtle differences in the initial Chk1-involved G(2) arrest with respect to p53/p21(WAF1) : absence of either protein led to late G(2) arrest instead of the classic G(2) arrest during checkpoint initiation, and this impacted the release back into the cell cycle.	topic_ccc
75367	2	355040	7	NULL	NULL	0	NULL	statement 1	Process		difference 		subtle			p53/p21(WAF1)	GP	with respect to			NULL		0	NULL	NULL	NULL	NULL	NULL	 We revealed subtle differences in the initial Chk1-involved G(2) arrest with respect to p53/p21(WAF1) : absence of either protein led to late G(2) arrest instead of the classic G(2) arrest during checkpoint initiation, and this impacted the release back into the cell cycle.	topic_ccc
75368	3	355040	7	NULL	NULL	0	NULL	Chk1	GP	absence of	leads to					late G(2) arrest	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 We revealed subtle differences in the initial Chk1-involved G(2) arrest with respect to p53/p21(WAF1) : absence of either protein led to late G(2) arrest instead of the classic G(2) arrest during checkpoint initiation, and this impacted the release back into the cell cycle.	topic_ccc
75369	4	355040	7	NULL	NULL	0	NULL	p53/p21(WAF1)	GP	absence of	leads to					late G(2) arrest	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 We revealed subtle differences in the initial Chk1-involved G(2) arrest with respect to p53/p21(WAF1) : absence of either protein led to late G(2) arrest instead of the classic G(2) arrest during checkpoint initiation, and this impacted the release back into the cell cycle.	topic_ccc
75370	5	355040	7	NULL	NULL	0	NULL	Chk1	GP	absence of	does not lead to					classic G(2) arrest	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 We revealed subtle differences in the initial Chk1-involved G(2) arrest with respect to p53/p21(WAF1) : absence of either protein led to late G(2) arrest instead of the classic G(2) arrest during checkpoint initiation, and this impacted the release back into the cell cycle.	topic_ccc
75371	6	355040	7	NULL	NULL	0	NULL	p53/p21(WAF1)	GP	absence of	does not lead to					classic G(2) arrest	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 We revealed subtle differences in the initial Chk1-involved G(2) arrest with respect to p53/p21(WAF1) : absence of either protein led to late G(2) arrest instead of the classic G(2) arrest during checkpoint initiation, and this impacted the release back into the cell cycle.	topic_ccc
75372	7	355040	7	NULL	NULL	0	NULL	statement 3	Process		occur during					checkpoint initiation	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 We revealed subtle differences in the initial Chk1-involved G(2) arrest with respect to p53/p21(WAF1) : absence of either protein led to late G(2) arrest instead of the classic G(2) arrest during checkpoint initiation, and this impacted the release back into the cell cycle.	topic_ccc
75373	8	355040	7	NULL	NULL	0	NULL	statement 4	Process		occur during					checkpoint initiation	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 We revealed subtle differences in the initial Chk1-involved G(2) arrest with respect to p53/p21(WAF1) : absence of either protein led to late G(2) arrest instead of the classic G(2) arrest during checkpoint initiation, and this impacted the release back into the cell cycle.	topic_ccc
75374	9	355040	7	NULL	NULL	0	NULL	statement 3	Process		impacts					cell cycle	Process	release back into the			NULL		0	NULL	NULL	NULL	NULL	NULL	 We revealed subtle differences in the initial Chk1-involved G(2) arrest with respect to p53/p21(WAF1) : absence of either protein led to late G(2) arrest instead of the classic G(2) arrest during checkpoint initiation, and this impacted the release back into the cell cycle.	topic_ccc
75375	10	355040	7	NULL	NULL	0	NULL	statement 4	Process		impacts					Cell cycle	Process	release back into the			NULL		0	NULL	NULL	NULL	NULL	NULL	 We revealed subtle differences in the initial Chk1-involved G(2) arrest with respect to p53/p21(WAF1) : absence of either protein led to late G(2) arrest instead of the classic G(2) arrest during checkpoint initiation, and this impacted the release back into the cell cycle.	topic_ccc
75518	1	355042	7	NULL	NULL	0	NULL	colorectal adenomas	MedicalFinding	reduced risk of	associated with					GH1	GP	homozygous variant genotype			NULL		0	NULL	NULL	NULL	NULL	NULL	There was a reduced risk of colorectal adenomas (OR=0.63, 95% CI 0.42-0.94) and hyperplastic polyps (OR=0.7, 95% CI 0.5-0.9) associated with the homozygous variant genotype for GH1.	topic_ccc
75519	2	355042	7	NULL	NULL	0	NULL	hyperplastic polyps	MedicalFinding	reduced risk of	associated with					GH1	GP	homozygous variant genotype			NULL		0	NULL	NULL	NULL	NULL	NULL	There was a reduced risk of colorectal adenomas (OR=0.63, 95% CI 0.42-0.94) and hyperplastic polyps (OR=0.7, 95% CI 0.5-0.9) associated with the homozygous variant genotype for GH1.	topic_ccc
75520	1	355043	7	NULL	NULL	0	NULL	Colon cancer	MedicalFinding		is a common type of					cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Colon cancer is a common type of cancer. A number of risk factors increase the likelihood of developing colon cancer. A risk factor is something that increases your likelihood of developing cancer.	topic_ccc
75521	1	355044	7	NULL	NULL	0	NULL	sweetened beverages	Food		concern in		potential			obesity	MedicalFinding	relation to risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	Some studies, specifically on sweetened beverages, highlighted a potential concern in relation to obesity risk, although these were limited by important methodological issues.	topic_ccc
75522	1	355045	7	NULL	NULL	0	NULL	HIF1A	GP	overexpression of	associated with		significantly			colorectal cancer-specific mortality 	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	 HIF1A overexpression was significantly associated with higher colorectal cancer-specific mortality in Kaplan-Meier analysis (log-rank test, P < 0.0001), univariate Cox regression (hazard ratio = 1.84; 95% confidence interval, 1.37 to 2.47; P < 0.0001) and multivariate analysis (adjusted hazard ratio = 1.72; 95% confidence interval, 1.26 to 2.36; P = 0.0007) that adjusted for clinical and tumoral features, including microsatellite instability, TP53 (p53), PTGS2 (cyclooxygenase-2), CpG island methylator phenotype, and KRAS, BRAF, PIK3CA, and LINE-1 methylation.	topic_ccc
75523	1	355046	7	NULL	NULL	0	NULL	HIF-1	GP		mediators of		essential			cellular response	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Hypoxia- inducible factor (HIF)-1 and HIF-2, which are essential mediators of cellular response to hypoxia, regulate gene expression for tumor angiogenesis, glucose metabolism, and resistance to oxidative stress. Their key regulatory subunits, HIF1A (HIF-1alpha) and endothelial PAS domain protein 1 (EPAS1; HIF-2alpha), are overexpressed and associated with patient prognosis in a variety of cancers.	topic_ccc
75524	2	355046	7	NULL	NULL	0	NULL	statement 1	Process		in response to					hypoxia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Hypoxia- inducible factor (HIF)-1 and HIF-2, which are essential mediators of cellular response to hypoxia, regulate gene expression for tumor angiogenesis, glucose metabolism, and resistance to oxidative stress. Their key regulatory subunits, HIF1A (HIF-1alpha) and endothelial PAS domain protein 1 (EPAS1; HIF-2alpha), are overexpressed and associated with patient prognosis in a variety of cancers.	topic_ccc
75525	3	355046	7	NULL	NULL	NULL	NULL	HIF-2	GP		mediators of		essential			 cellular response	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hypoxia- inducible factor (HIF)-1 and HIF-2, which are essential mediators of cellular response to hypoxia, regulate gene expression for tumor angiogenesis, glucose metabolism, and resistance to oxidative stress. Their key regulatory subunits, HIF1A (HIF-1alpha) and endothelial PAS domain protein 1 (EPAS1; HIF-2alpha), are overexpressed and associated with patient prognosis in a variety of cancers.	topic_ccc
75526	4	355046	7	NULL	NULL	0	NULL	statement 3	Process		in response to					hypoxia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Hypoxia- inducible factor (HIF)-1 and HIF-2, which are essential mediators of cellular response to hypoxia, regulate gene expression for tumor angiogenesis, glucose metabolism, and resistance to oxidative stress. Their key regulatory subunits, HIF1A (HIF-1alpha) and endothelial PAS domain protein 1 (EPAS1; HIF-2alpha), are overexpressed and associated with patient prognosis in a variety of cancers.	topic_ccc
75527	5	355046	7	NULL	NULL	0	NULL	HIF-1	GP		regulate					gene expression	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Hypoxia- inducible factor (HIF)-1 and HIF-2, which are essential mediators of cellular response to hypoxia, regulate gene expression for tumor angiogenesis, glucose metabolism, and resistance to oxidative stress. Their key regulatory subunits, HIF1A (HIF-1alpha) and endothelial PAS domain protein 1 (EPAS1; HIF-2alpha), are overexpressed and associated with patient prognosis in a variety of cancers.	topic_ccc
75528	6	355046	7	NULL	NULL	0	NULL	HIF-2	GP		regulate					gene expression	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Hypoxia- inducible factor (HIF)-1 and HIF-2, which are essential mediators of cellular response to hypoxia, regulate gene expression for tumor angiogenesis, glucose metabolism, and resistance to oxidative stress. Their key regulatory subunits, HIF1A (HIF-1alpha) and endothelial PAS domain protein 1 (EPAS1; HIF-2alpha), are overexpressed and associated with patient prognosis in a variety of cancers.	topic_ccc
75529	7	355046	7	NULL	NULL	0	NULL	statement 5	Process		occur for					tumor angiogenesis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Hypoxia- inducible factor (HIF)-1 and HIF-2, which are essential mediators of cellular response to hypoxia, regulate gene expression for tumor angiogenesis, glucose metabolism, and resistance to oxidative stress. Their key regulatory subunits, HIF1A (HIF-1alpha) and endothelial PAS domain protein 1 (EPAS1; HIF-2alpha), are overexpressed and associated with patient prognosis in a variety of cancers.	topic_ccc
75530	8	355046	7	NULL	NULL	0	NULL	statement 6	Process		occur for					tumor angiogenesis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Hypoxia- inducible factor (HIF)-1 and HIF-2, which are essential mediators of cellular response to hypoxia, regulate gene expression for tumor angiogenesis, glucose metabolism, and resistance to oxidative stress. Their key regulatory subunits, HIF1A (HIF-1alpha) and endothelial PAS domain protein 1 (EPAS1; HIF-2alpha), are overexpressed and associated with patient prognosis in a variety of cancers.	topic_ccc
75531	9	355046	7	NULL	NULL	0	NULL	statement 5	Process		occur for					glucose metabolism	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Hypoxia- inducible factor (HIF)-1 and HIF-2, which are essential mediators of cellular response to hypoxia, regulate gene expression for tumor angiogenesis, glucose metabolism, and resistance to oxidative stress. Their key regulatory subunits, HIF1A (HIF-1alpha) and endothelial PAS domain protein 1 (EPAS1; HIF-2alpha), are overexpressed and associated with patient prognosis in a variety of cancers.	topic_ccc
75532	10	355046	7	NULL	NULL	0	NULL	statement 6	Process		occur for					glucose metabolism	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Hypoxia- inducible factor (HIF)-1 and HIF-2, which are essential mediators of cellular response to hypoxia, regulate gene expression for tumor angiogenesis, glucose metabolism, and resistance to oxidative stress. Their key regulatory subunits, HIF1A (HIF-1alpha) and endothelial PAS domain protein 1 (EPAS1; HIF-2alpha), are overexpressed and associated with patient prognosis in a variety of cancers.	topic_ccc
75533	11	355046	7	NULL	NULL	0	NULL	statement 5	Process		occur for					oxidative stress	Process	resistance to			NULL		0	NULL	NULL	NULL	NULL	NULL	Hypoxia- inducible factor (HIF)-1 and HIF-2, which are essential mediators of cellular response to hypoxia, regulate gene expression for tumor angiogenesis, glucose metabolism, and resistance to oxidative stress. Their key regulatory subunits, HIF1A (HIF-1alpha) and endothelial PAS domain protein 1 (EPAS1; HIF-2alpha), are overexpressed and associated with patient prognosis in a variety of cancers.	topic_ccc
75534	12	355046	7	NULL	NULL	0	NULL	statement 6	Process		occur for					oxidative stress	Process	resistance to			NULL		0	NULL	NULL	NULL	NULL	NULL	Hypoxia- inducible factor (HIF)-1 and HIF-2, which are essential mediators of cellular response to hypoxia, regulate gene expression for tumor angiogenesis, glucose metabolism, and resistance to oxidative stress. Their key regulatory subunits, HIF1A (HIF-1alpha) and endothelial PAS domain protein 1 (EPAS1; HIF-2alpha), are overexpressed and associated with patient prognosis in a variety of cancers.	topic_ccc
75535	13	355046	7	NULL	NULL	NULL	NULL	HIF1A	GP		 subunit of		regulatory			HIF-1	GP				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hypoxia- inducible factor (HIF)-1 and HIF-2, which are essential mediators of cellular response to hypoxia, regulate gene expression for tumor angiogenesis, glucose metabolism, and resistance to oxidative stress. Their key regulatory subunits, HIF1A (HIF-1alpha) and endothelial PAS domain protein 1 (EPAS1; HIF-2alpha), are overexpressed and associated with patient prognosis in a variety of cancers.	topic_ccc
75536	14	355046	7	NULL	NULL	0	NULL	HIF1A	GP	overexpression of	associated with					cancers	MedicalFinding	prognosis in			NULL		0	NULL	NULL	NULL	NULL	NULL	Hypoxia- inducible factor (HIF)-1 and HIF-2, which are essential mediators of cellular response to hypoxia, regulate gene expression for tumor angiogenesis, glucose metabolism, and resistance to oxidative stress. Their key regulatory subunits, HIF1A (HIF-1alpha) and endothelial PAS domain protein 1 (EPAS1; HIF-2alpha), are overexpressed and associated with patient prognosis in a variety of cancers.	topic_ccc
75537	15	355046	7	NULL	NULL	NULL	NULL	EPAS1	GP		subunit of		regulatory			HIF-2	GP				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hypoxia- inducible factor (HIF)-1 and HIF-2, which are essential mediators of cellular response to hypoxia, regulate gene expression for tumor angiogenesis, glucose metabolism, and resistance to oxidative stress. Their key regulatory subunits, HIF1A (HIF-1alpha) and endothelial PAS domain protein 1 (EPAS1; HIF-2alpha), are overexpressed and associated with patient prognosis in a variety of cancers.	topic_ccc
75538	16	355046	7	NULL	NULL	0	NULL	EPAS1	GP	overexpression of	associated with					cancers	MedicalFinding	prognosis in			NULL		0	NULL	NULL	NULL	NULL	NULL	Hypoxia- inducible factor (HIF)-1 and HIF-2, which are essential mediators of cellular response to hypoxia, regulate gene expression for tumor angiogenesis, glucose metabolism, and resistance to oxidative stress. Their key regulatory subunits, HIF1A (HIF-1alpha) and endothelial PAS domain protein 1 (EPAS1; HIF-2alpha), are overexpressed and associated with patient prognosis in a variety of cancers.	topic_ccc
75539	17	355046	7	NULL	NULL	0	NULL	HIF1A	GP		is					HIF-1alpha	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Hypoxia- inducible factor (HIF)-1 and HIF-2, which are essential mediators of cellular response to hypoxia, regulate gene expression for tumor angiogenesis, glucose metabolism, and resistance to oxidative stress. Their key regulatory subunits, HIF1A (HIF-1alpha) and endothelial PAS domain protein 1 (EPAS1; HIF-2alpha), are overexpressed and associated with patient prognosis in a variety of cancers.	topic_ccc
75540	18	355046	7	NULL	NULL	0	NULL	EPAS1	GP		is					endothelial PAS domain protein 1 	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Hypoxia- inducible factor (HIF)-1 and HIF-2, which are essential mediators of cellular response to hypoxia, regulate gene expression for tumor angiogenesis, glucose metabolism, and resistance to oxidative stress. Their key regulatory subunits, HIF1A (HIF-1alpha) and endothelial PAS domain protein 1 (EPAS1; HIF-2alpha), are overexpressed and associated with patient prognosis in a variety of cancers.	topic_ccc
75541	1	355047	7	NULL	NULL	NULL	NULL	HIF1A 	GP	expression of	associated with		independently			colorectal cancer	MedicalFinding	poor prognosis in			NULL		NULL	NULL	NULL	NULL	NULL	NULL	 In conclusion, HIF1A expression is independently associated with poor prognosis in colorectal cancer, suggesting HIF1A as a biomarker with potentially important therapeutic implications.	topic_ccc
75542	2	355047	7	NULL	NULL	0	NULL	HIF1A	GP		biomarker with		potential			therapeutic implications	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	 In conclusion, HIF1A expression is independently associated with poor prognosis in colorectal cancer, suggesting HIF1A as a biomarker with potentially important therapeutic implications.	topic_ccc
75543	3	355047	7	NULL	NULL	0	NULL	statement 1	Process		suggest					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 In conclusion, HIF1A expression is independently associated with poor prognosis in colorectal cancer, suggesting HIF1A as a biomarker with potentially important therapeutic implications.	topic_ccc
75544	1	355048	7	NULL	NULL	0	NULL	IGF-IR	GP	signaling of	is required for					carcinogenicity	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-like growth factor (IGF)-I receptor (IGF-IR) signaling is required for carcinogenicity and proliferation of gastrointestinal cancers.	topic_ccc
75545	2	355048	7	NULL	NULL	0	NULL	IGF-IR	GP	signaling of	is required for					gastrointestinal cancers	MedicalFinding	proliferation of			NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-like growth factor (IGF)-I receptor (IGF-IR) signaling is required for carcinogenicity and proliferation of gastrointestinal cancers.	topic_ccc
75546	3	355048	7	NULL	NULL	0	NULL	IGF-IR	GP		is					Insulin-like growth factor-I receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-like growth factor (IGF)-I receptor (IGF-IR) signaling is required for carcinogenicity and proliferation of gastrointestinal cancers.	topic_ccc
75547	1	355049	7	NULL	NULL	0	NULL	IGF-1	GP		is critical to					inflammatory response	MedicalFinding	activate			NULL	liver	0	NULL	NULL	NULL	NULL	NULL	In the setting of obesity, our findings imply that IGF-1 is critical to activate and sustain an inflammatory response in the liver that is needed for hepatic metastasis, not only through direct, paracrine effect on tumor cell growth, but also through indirect effects involving the tumor microenvironment.	topic_ccc
75548	2	355049	7	NULL	NULL	0	NULL	IGF-1	GP		is critical to					inflammatory response	MedicalFinding	sustain			NULL	liver	0	NULL	NULL	NULL	NULL	NULL	In the setting of obesity, our findings imply that IGF-1 is critical to activate and sustain an inflammatory response in the liver that is needed for hepatic metastasis, not only through direct, paracrine effect on tumor cell growth, but also through indirect effects involving the tumor microenvironment.	topic_ccc
75549	3	355049	7	NULL	NULL	0	NULL	statement 1	Process		occur along with					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	In the setting of obesity, our findings imply that IGF-1 is critical to activate and sustain an inflammatory response in the liver that is needed for hepatic metastasis, not only through direct, paracrine effect on tumor cell growth, but also through indirect effects involving the tumor microenvironment.	topic_ccc
75550	4	355049	7	NULL	NULL	0	NULL	statement 3	Process		required for					hepatic metastasis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	In the setting of obesity, our findings imply that IGF-1 is critical to activate and sustain an inflammatory response in the liver that is needed for hepatic metastasis, not only through direct, paracrine effect on tumor cell growth, but also through indirect effects involving the tumor microenvironment.	topic_ccc
75551	5	355049	7	NULL	NULL	NULL	NULL	statement 4	Process		occur through		directly			tumor cell growth	Process	paracrine effect on			NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the setting of obesity, our findings imply that IGF-1 is critical to activate and sustain an inflammatory response in the liver that is needed for hepatic metastasis, not only through direct, paracrine effect on tumor cell growth, but also through indirect effects involving the tumor microenvironment.	topic_ccc
75552	6	355049	7	NULL	NULL	0	NULL	statement 4	Process		occur through		indirectly			tumor microenvironment	Process	effects involving			NULL		0	NULL	NULL	NULL	NULL	NULL	In the setting of obesity, our findings imply that IGF-1 is critical to activate and sustain an inflammatory response in the liver that is needed for hepatic metastasis, not only through direct, paracrine effect on tumor cell growth, but also through indirect effects involving the tumor microenvironment.	topic_ccc
75553	1	355050	7	NULL	NULL	0	NULL	IL-12	GP		role in		prominent			TH1 T cell differentiation	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The prominent role of interleukin (IL)-12 in inflammatory responses, especially in TH1 T cell differentiation, is well established.	topic_ccc
75554	2	355050	7	NULL	NULL	0	NULL	TH1 T cell differentiation	Process		is a type of					 inflammatory response	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The prominent role of interleukin (IL)-12 in inflammatory responses, especially in TH1 T cell differentiation, is well established.	topic_ccc
75555	3	355050	7	NULL	NULL	0	NULL	IL-12	GP		is					Interleukin-12	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The prominent role of interleukin (IL)-12 in inflammatory responses, especially in TH1 T cell differentiation, is well established.	topic_ccc
74084	1	355052	5	NULL	NULL	0	NULL	siblings of schizophrenia patients	GroupOfPeople		experience					impaired cognition	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Siblings of patients with schizophrenia show impaired cognition and an increased prevalence of depression history.	topic_sch
74085	2	355052	5	NULL	NULL	0	NULL	siblings of schizophrenia patients	GroupOfPeople		experience					depression	MedicalFinding	increased prevalence of;;history of			NULL		0	NULL	NULL	NULL	NULL	NULL	Siblings of patients with schizophrenia show impaired cognition and an increased prevalence of depression history.	topic_sch
74144	1	355053	5	NULL	NULL	0	NULL	KYNA	Chemical		is					kynurenic acid	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Kynurenic acid (KYNA) is an endogenous tryptophan-metabolite found to be increased in the brain of patients with schizophrenia ([Erhardt et al., 2009] and [Wonodi and Schwarcz, 2010])	topic_sch
74145	2	355053	5	NULL	NULL	0	NULL	Kynurenic acid	Chemical		is a type of					endogenous tryptophan-metabolite 	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Kynurenic acid (KYNA) is an endogenous tryptophan-metabolite found to be increased in the brain of patients with schizophrenia ([Erhardt et al., 2009] and [Wonodi and Schwarcz, 2010])	topic_sch
74146	3	355053	5	NULL	NULL	0	NULL	Kynurenic acid	Chemical		is increased in					schizophrenia patients	GroupOfPeople	brain of			NULL		0	NULL	NULL	NULL	NULL	NULL	Kynurenic acid (KYNA) is an endogenous tryptophan-metabolite found to be increased in the brain of patients with schizophrenia ([Erhardt et al., 2009] and [Wonodi and Schwarcz, 2010])	topic_sch
74147	1	355054	5	NULL	NULL	0	NULL	hypoglutamatergia	MedicalFinding		is implicated in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	This unique receptor profile may account for both hypoglutamatergia and impairment in cholinergic signaling, conditions that are implicated in schizophrenia (Wonodi and Schwarcz, 2010).	topic_sch
74148	2	355054	5	NULL	NULL	0	NULL	cholinergic signaling	Process	impairment of	is implicated in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	This unique receptor profile may account for both hypoglutamatergia and impairment in cholinergic signaling, conditions that are implicated in schizophrenia (Wonodi and Schwarcz, 2010).	topic_sch
74149	1	355055	5	NULL	NULL	0	NULL	KMO gene	GP		is located on					1q42	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	Notably, the KMO gene is located on 1q42, a chromosome region associated with schizophrenia ([Ekelund et al., 2004] and [Hamshere et al., 2005]).	topic_sch
74150	2	355055	5	NULL	NULL	0	NULL	1q42	Chromosome		is associated with					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Notably, the KMO gene is located on 1q42, a chromosome region associated with schizophrenia ([Ekelund et al., 2004] and [Hamshere et al., 2005]).	topic_sch
74151	1	355056	5	NULL	NULL	0	NULL	KMO variations	GP		is associated with		may be			schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Here, we investigate a possible association between KMO variations and schizophrenia.	topic_sch
74152	1	355057	5	NULL	NULL	0	NULL	KYNA	GP	synthesis of;;brain	is dependent on					kynurenine	GP	availability of			NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore, beyond the activity of KMO, the synthesis of brain KYNA is also highly dependent on the availability of kynurenine, the immediate precursor of KYNA. As recent studies show that also kynurenine is elevated in patients with schizophrenia ([Linderholm et al., in press] and [Wonodi and Schwarcz, 2010]), one may speculate that polymorphisms in genes encoding indoleamine 2,3-dioxygenase (IDO) and/or tryptophan 2,3-dioxygenase (TDO), enzymes converting tryptophan to kynurenine, may partly account for the elevated levels of KYNA in schizophrenia.	topic_sch
74153	2	355057	5	NULL	NULL	0	NULL	kynurenine	GP		is an immediate precursor of					KYNA	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore, beyond the activity of KMO, the synthesis of brain KYNA is also highly dependent on the availability of kynurenine, the immediate precursor of KYNA. As recent studies show that also kynurenine is elevated in patients with schizophrenia ([Linderholm et al., in press] and [Wonodi and Schwarcz, 2010]), one may speculate that polymorphisms in genes encoding indoleamine 2,3-dioxygenase (IDO) and/or tryptophan 2,3-dioxygenase (TDO), enzymes converting tryptophan to kynurenine, may partly account for the elevated levels of KYNA in schizophrenia.	topic_sch
74154	3	355057	5	NULL	NULL	0	NULL	kynurenine	GP		is elevated in					schizophrenic patients	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore, beyond the activity of KMO, the synthesis of brain KYNA is also highly dependent on the availability of kynurenine, the immediate precursor of KYNA. As recent studies show that also kynurenine is elevated in patients with schizophrenia ([Linderholm et al., in press] and [Wonodi and Schwarcz, 2010]), one may speculate that polymorphisms in genes encoding indoleamine 2,3-dioxygenase (IDO) and/or tryptophan 2,3-dioxygenase (TDO), enzymes converting tryptophan to kynurenine, may partly account for the elevated levels of KYNA in schizophrenia.	topic_sch
74155	4	355057	5	NULL	NULL	0	NULL	tryptophan	AminoAcid		is converted to					kynurenine	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore, beyond the activity of KMO, the synthesis of brain KYNA is also highly dependent on the availability of kynurenine, the immediate precursor of KYNA. As recent studies show that also kynurenine is elevated in patients with schizophrenia ([Linderholm et al., in press] and [Wonodi and Schwarcz, 2010]), one may speculate that polymorphisms in genes encoding indoleamine 2,3-dioxygenase (IDO) and/or tryptophan 2,3-dioxygenase (TDO), enzymes converting tryptophan to kynurenine, may partly account for the elevated levels of KYNA in schizophrenia.	topic_sch
74156	5	355057	5	NULL	NULL	0	NULL	enzymes	GP		is required for					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore, beyond the activity of KMO, the synthesis of brain KYNA is also highly dependent on the availability of kynurenine, the immediate precursor of KYNA. As recent studies show that also kynurenine is elevated in patients with schizophrenia ([Linderholm et al., in press] and [Wonodi and Schwarcz, 2010]), one may speculate that polymorphisms in genes encoding indoleamine 2,3-dioxygenase (IDO) and/or tryptophan 2,3-dioxygenase (TDO), enzymes converting tryptophan to kynurenine, may partly account for the elevated levels of KYNA in schizophrenia.	topic_sch
74157	6	355057	5	NULL	NULL	0	NULL	statement 5	Process		accounts for		partly			statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore, beyond the activity of KMO, the synthesis of brain KYNA is also highly dependent on the availability of kynurenine, the immediate precursor of KYNA. As recent studies show that also kynurenine is elevated in patients with schizophrenia ([Linderholm et al., in press] and [Wonodi and Schwarcz, 2010]), one may speculate that polymorphisms in genes encoding indoleamine 2,3-dioxygenase (IDO) and/or tryptophan 2,3-dioxygenase (TDO), enzymes converting tryptophan to kynurenine, may partly account for the elevated levels of KYNA in schizophrenia.	topic_sch
74158	7	355057	5	NULL	NULL	0	NULL	IDO	GP		is					indoleamine 2,3-dioxygenase	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore, beyond the activity of KMO, the synthesis of brain KYNA is also highly dependent on the availability of kynurenine, the immediate precursor of KYNA. As recent studies show that also kynurenine is elevated in patients with schizophrenia ([Linderholm et al., in press] and [Wonodi and Schwarcz, 2010]), one may speculate that polymorphisms in genes encoding indoleamine 2,3-dioxygenase (IDO) and/or tryptophan 2,3-dioxygenase (TDO), enzymes converting tryptophan to kynurenine, may partly account for the elevated levels of KYNA in schizophrenia.	topic_sch
74159	8	355057	5	NULL	NULL	0	NULL	TDO	GP		is					tryptophan 2,3-dioxygenase	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore, beyond the activity of KMO, the synthesis of brain KYNA is also highly dependent on the availability of kynurenine, the immediate precursor of KYNA. As recent studies show that also kynurenine is elevated in patients with schizophrenia ([Linderholm et al., in press] and [Wonodi and Schwarcz, 2010]), one may speculate that polymorphisms in genes encoding indoleamine 2,3-dioxygenase (IDO) and/or tryptophan 2,3-dioxygenase (TDO), enzymes converting tryptophan to kynurenine, may partly account for the elevated levels of KYNA in schizophrenia.	topic_sch
74160	9	355057	5	NULL	NULL	0	NULL	IDO gene	GP	polymorphism of	accounts for		partly			statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore, beyond the activity of KMO, the synthesis of brain KYNA is also highly dependent on the availability of kynurenine, the immediate precursor of KYNA. As recent studies show that also kynurenine is elevated in patients with schizophrenia ([Linderholm et al., in press] and [Wonodi and Schwarcz, 2010]), one may speculate that polymorphisms in genes encoding indoleamine 2,3-dioxygenase (IDO) and/or tryptophan 2,3-dioxygenase (TDO), enzymes converting tryptophan to kynurenine, may partly account for the elevated levels of KYNA in schizophrenia.	topic_sch
74161	10	355057	5	NULL	NULL	0	NULL	TDO gene	GP	polymorphism of	accounts for		partly			statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore, beyond the activity of KMO, the synthesis of brain KYNA is also highly dependent on the availability of kynurenine, the immediate precursor of KYNA. As recent studies show that also kynurenine is elevated in patients with schizophrenia ([Linderholm et al., in press] and [Wonodi and Schwarcz, 2010]), one may speculate that polymorphisms in genes encoding indoleamine 2,3-dioxygenase (IDO) and/or tryptophan 2,3-dioxygenase (TDO), enzymes converting tryptophan to kynurenine, may partly account for the elevated levels of KYNA in schizophrenia.	topic_sch
74162	1	355058	5	NULL	NULL	0	NULL	cannabis abuse	MedicalFinding	prevalence of	is increased in					schizophrenic patients	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with schizophrenia show increased prevalence of cannabis abuse and this has been linked to severity of EPS.	topic_sch
74163	2	355058	5	NULL	NULL	0	NULL	statement 1	Process		is linked to					EPS	MedicalFinding	severity of			NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with schizophrenia show increased prevalence of cannabis abuse and this has been linked to severity of EPS.	topic_sch
74164	1	355059	5	NULL	NULL	0	NULL	mitochondrial dysfunction	MedicalFinding		occurs in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Alterations in mitochondrial morphometry, brain energy metabolism, and enzymatic activity in the mitochondrial respiratory chain suggest a mitochondrial dysfunction in schizophrenia that could be related to the genetic characteristics of mtDNA. 	topic_sch
74165	2	355059	5	NULL	NULL	0	NULL	statement 1	Process		is related to					mtDNA	NucleicAcid	genetic characteristics of			NULL		0	NULL	NULL	NULL	NULL	NULL	Alterations in mitochondrial morphometry, brain energy metabolism, and enzymatic activity in the mitochondrial respiratory chain suggest a mitochondrial dysfunction in schizophrenia that could be related to the genetic characteristics of mtDNA. 	topic_sch
74166	3	355059	5	NULL	NULL	NULL	NULL	mitochondrial morphometry	QuantityOrMeasure	alterations in	suggest					statement 1	Process				NULL	mitochondrial respiratory chain	NULL	NULL	NULL	NULL	NULL	NULL	Alterations in mitochondrial morphometry, brain energy metabolism, and enzymatic activity in the mitochondrial respiratory chain suggest a mitochondrial dysfunction in schizophrenia that could be related to the genetic characteristics of mtDNA. 	topic_sch
74167	4	355059	5	NULL	NULL	NULL	NULL	brain energy metabolism	Process	alterations in	suggest					statement 1	Process				NULL	mitochondrial respiratory chain	NULL	NULL	NULL	NULL	NULL	NULL	Alterations in mitochondrial morphometry, brain energy metabolism, and enzymatic activity in the mitochondrial respiratory chain suggest a mitochondrial dysfunction in schizophrenia that could be related to the genetic characteristics of mtDNA. 	topic_sch
74168	5	355059	5	NULL	NULL	NULL	NULL	enzymatic activity	Process	alterations in	suggest					statement 1	Process				NULL	mitochondrial respiratory chain	NULL	NULL	NULL	NULL	NULL	NULL	Alterations in mitochondrial morphometry, brain energy metabolism, and enzymatic activity in the mitochondrial respiratory chain suggest a mitochondrial dysfunction in schizophrenia that could be related to the genetic characteristics of mtDNA. 	topic_sch
74169	1	355060	5	NULL	NULL	0	NULL	mtDNA	NucleicAcid		is involved in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, evidence of maternal inheritance and the presence of schizophrenia symptoms in patients suffering from a mitochondrial disorder related to an mtDNA mutation suggest that mtDNA is involved in schizophrenia	topic_sch
74170	2	355060	5	NULL	NULL	0	NULL	mitochondrial disorder	MedicalFinding		is related to					mtDNA	NucleicAcid	mutation of			NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, evidence of maternal inheritance and the presence of schizophrenia symptoms in patients suffering from a mitochondrial disorder related to an mtDNA mutation suggest that mtDNA is involved in schizophrenia	topic_sch
74171	3	355060	5	NULL	NULL	NULL	NULL	maternal inheritance	Process		is evident in					mitochondrial disorder	MedicalFinding	patients of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Moreover, evidence of maternal inheritance and the presence of schizophrenia symptoms in patients suffering from a mitochondrial disorder related to an mtDNA mutation suggest that mtDNA is involved in schizophrenia	topic_sch
74172	4	355060	5	NULL	NULL	0	NULL	schizophrenia	MedicalFinding	presence of;;symptoms of	is present in					mitochondrial disorder	MedicalFinding	patients of			NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, evidence of maternal inheritance and the presence of schizophrenia symptoms in patients suffering from a mitochondrial disorder related to an mtDNA mutation suggest that mtDNA is involved in schizophrenia	topic_sch
75556	1	355062	7	NULL	NULL	0	NULL	Bipolar I disorder	MedicalFinding		sub-diagnosis of					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar I disorder is a sub-diagnosis of bipolar disorder that is characterized by at least one manic or mixed episode.	topic_bd
75557	2	355062	7	NULL	NULL	0	NULL	Bipolar I disorder	MedicalFinding		is characterized by					manic episode	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar I disorder is a sub-diagnosis of bipolar disorder that is characterized by at least one manic or mixed episode.	topic_bd
75558	3	355062	7	NULL	NULL	0	NULL	Bipolar I disorder	MedicalFinding		is characterized by					mixed episode	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar I disorder is a sub-diagnosis of bipolar disorder that is characterized by at least one manic or mixed episode.	topic_bd
75559	4	355062	7	NULL	NULL	0	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar I disorder is a sub-diagnosis of bipolar disorder that is characterized by at least one manic or mixed episode.	topic_bd
75413	1	355063	11	NULL	NULL	0	NULL	hlorhexidine	Chemical		is a type of 					chemical antiseptic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	hlorhexidine is a chemical antiseptic. It is effective on both Gram-positive and Gram-negative bacteria, although it is less effective with some Gram-negative bacteria. It has both bactericidal as well as bacteriostatic mechanisms of action,	topic_mrs
75414	2	355063	11	NULL	NULL	0	NULL	hlorhexidine	Chemical		is effective on					Gram-positive bacteria	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	hlorhexidine is a chemical antiseptic. It is effective on both Gram-positive and Gram-negative bacteria, although it is less effective with some Gram-negative bacteria. It has both bactericidal as well as bacteriostatic mechanisms of action,	topic_mrs
75415	3	355063	11	NULL	NULL	0	NULL	hlorhexidine	Chemical		is effective on		may			Gram-negative bacteria	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	hlorhexidine is a chemical antiseptic. It is effective on both Gram-positive and Gram-negative bacteria, although it is less effective with some Gram-negative bacteria. It has both bactericidal as well as bacteriostatic mechanisms of action,	topic_mrs
75416	4	355063	11	NULL	NULL	0	NULL	hlorhexidine	Chemical		acts as					bactericidal 	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	hlorhexidine is a chemical antiseptic. It is effective on both Gram-positive and Gram-negative bacteria, although it is less effective with some Gram-negative bacteria. It has both bactericidal as well as bacteriostatic mechanisms of action,	topic_mrs
75417	5	355063	11	NULL	NULL	0	NULL	hlorhexidine	Chemical		acts as					bacteriostatic	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	hlorhexidine is a chemical antiseptic. It is effective on both Gram-positive and Gram-negative bacteria, although it is less effective with some Gram-negative bacteria. It has both bactericidal as well as bacteriostatic mechanisms of action,	topic_mrs
75418	1	355065	11	NULL	NULL	0	NULL	 tea tree oil	Chemical		is a type of 					 antiseptic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Proponents believe tea tree oil is an antiseptic and use it to fight germs. It has been used to treat cuts, minor burns, athlete's foot, and insect bites. Some claim it can treat bacterial and fungal skin infections, wound infections, gum infections, acne, head lice, eczema, vaginal yeast infections, colds, pneumonia, and other respiratory illnesses.	topic_mrs
75419	2	355065	11	NULL	NULL	0	NULL	tea tree oil	Chemical		use to 					fight germs	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Proponents believe tea tree oil is an antiseptic and use it to fight germs. It has been used to treat cuts, minor burns, athlete's foot, and insect bites. Some claim it can treat bacterial and fungal skin infections, wound infections, gum infections, acne, head lice, eczema, vaginal yeast infections, colds, pneumonia, and other respiratory illnesses.	topic_mrs
75420	3	355065	11	NULL	NULL	0	NULL	tea tree oil	Chemical		 treat					cuts	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Proponents believe tea tree oil is an antiseptic and use it to fight germs. It has been used to treat cuts, minor burns, athlete's foot, and insect bites. Some claim it can treat bacterial and fungal skin infections, wound infections, gum infections, acne, head lice, eczema, vaginal yeast infections, colds, pneumonia, and other respiratory illnesses.	topic_mrs
75421	4	355065	11	NULL	NULL	0	NULL	tea tree oil	Chemical		treats					minor burns	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Proponents believe tea tree oil is an antiseptic and use it to fight germs. It has been used to treat cuts, minor burns, athlete's foot, and insect bites. Some claim it can treat bacterial and fungal skin infections, wound infections, gum infections, acne, head lice, eczema, vaginal yeast infections, colds, pneumonia, and other respiratory illnesses.	topic_mrs
75422	5	355065	11	NULL	NULL	0	NULL	tea tree oil	Chemical		treats					athlete's foot	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Proponents believe tea tree oil is an antiseptic and use it to fight germs. It has been used to treat cuts, minor burns, athlete's foot, and insect bites. Some claim it can treat bacterial and fungal skin infections, wound infections, gum infections, acne, head lice, eczema, vaginal yeast infections, colds, pneumonia, and other respiratory illnesses.	topic_mrs
75423	6	355065	11	NULL	NULL	0	NULL	tea tree oil	Chemical		treats					insect bites	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Proponents believe tea tree oil is an antiseptic and use it to fight germs. It has been used to treat cuts, minor burns, athlete's foot, and insect bites. Some claim it can treat bacterial and fungal skin infections, wound infections, gum infections, acne, head lice, eczema, vaginal yeast infections, colds, pneumonia, and other respiratory illnesses.	topic_mrs
75424	7	355065	11	NULL	NULL	0	NULL	tea tree oil	Chemical		treat		may			skin infections	Process	bacterial;;fungal 			NULL		0	NULL	NULL	NULL	NULL	NULL	Proponents believe tea tree oil is an antiseptic and use it to fight germs. It has been used to treat cuts, minor burns, athlete's foot, and insect bites. Some claim it can treat bacterial and fungal skin infections, wound infections, gum infections, acne, head lice, eczema, vaginal yeast infections, colds, pneumonia, and other respiratory illnesses.	topic_mrs
75425	8	355065	11	NULL	NULL	0	NULL	tea tree oil	Chemical		treats		may			wound infections	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Proponents believe tea tree oil is an antiseptic and use it to fight germs. It has been used to treat cuts, minor burns, athlete's foot, and insect bites. Some claim it can treat bacterial and fungal skin infections, wound infections, gum infections, acne, head lice, eczema, vaginal yeast infections, colds, pneumonia, and other respiratory illnesses.	topic_mrs
75426	9	355065	11	NULL	NULL	0	NULL	tea tree oil	Chemical		treats		may			 gum infections	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Proponents believe tea tree oil is an antiseptic and use it to fight germs. It has been used to treat cuts, minor burns, athlete's foot, and insect bites. Some claim it can treat bacterial and fungal skin infections, wound infections, gum infections, acne, head lice, eczema, vaginal yeast infections, colds, pneumonia, and other respiratory illnesses.	topic_mrs
75427	10	355065	11	NULL	NULL	0	NULL	tea tree oil	Chemical		treats		may			 acne	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Proponents believe tea tree oil is an antiseptic and use it to fight germs. It has been used to treat cuts, minor burns, athlete's foot, and insect bites. Some claim it can treat bacterial and fungal skin infections, wound infections, gum infections, acne, head lice, eczema, vaginal yeast infections, colds, pneumonia, and other respiratory illnesses.	topic_mrs
75428	11	355065	11	NULL	NULL	0	NULL	tea tree oil	Chemical		treats		may			head lice	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Proponents believe tea tree oil is an antiseptic and use it to fight germs. It has been used to treat cuts, minor burns, athlete's foot, and insect bites. Some claim it can treat bacterial and fungal skin infections, wound infections, gum infections, acne, head lice, eczema, vaginal yeast infections, colds, pneumonia, and other respiratory illnesses.	topic_mrs
75429	12	355065	11	NULL	NULL	0	NULL	tea tree oil	Chemical		treats		may			eczema	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Proponents believe tea tree oil is an antiseptic and use it to fight germs. It has been used to treat cuts, minor burns, athlete's foot, and insect bites. Some claim it can treat bacterial and fungal skin infections, wound infections, gum infections, acne, head lice, eczema, vaginal yeast infections, colds, pneumonia, and other respiratory illnesses.	topic_mrs
75430	13	355065	11	NULL	NULL	0	NULL	tea tree oil	Chemical		treats		may			vaginal infections	Process	 yeast 			NULL		0	NULL	NULL	NULL	NULL	NULL	Proponents believe tea tree oil is an antiseptic and use it to fight germs. It has been used to treat cuts, minor burns, athlete's foot, and insect bites. Some claim it can treat bacterial and fungal skin infections, wound infections, gum infections, acne, head lice, eczema, vaginal yeast infections, colds, pneumonia, and other respiratory illnesses.	topic_mrs
75431	14	355065	11	NULL	NULL	0	NULL	tea tree oil	Chemical		treats		may			colds	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Proponents believe tea tree oil is an antiseptic and use it to fight germs. It has been used to treat cuts, minor burns, athlete's foot, and insect bites. Some claim it can treat bacterial and fungal skin infections, wound infections, gum infections, acne, head lice, eczema, vaginal yeast infections, colds, pneumonia, and other respiratory illnesses.	topic_mrs
75432	15	355065	11	NULL	NULL	0	NULL	tea tree oil	Chemical		treats		may			pneumonia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Proponents believe tea tree oil is an antiseptic and use it to fight germs. It has been used to treat cuts, minor burns, athlete's foot, and insect bites. Some claim it can treat bacterial and fungal skin infections, wound infections, gum infections, acne, head lice, eczema, vaginal yeast infections, colds, pneumonia, and other respiratory illnesses.	topic_mrs
75433	16	355065	11	NULL	NULL	0	NULL	tea tree oil	Chemical		treats		may			respiratory illnesses	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Proponents believe tea tree oil is an antiseptic and use it to fight germs. It has been used to treat cuts, minor burns, athlete's foot, and insect bites. Some claim it can treat bacterial and fungal skin infections, wound infections, gum infections, acne, head lice, eczema, vaginal yeast infections, colds, pneumonia, and other respiratory illnesses.	topic_mrs
74173	1	355066	5	NULL	NULL	0	NULL	savantism	MedicalFinding		is a form of					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	People with a form of autism, called savantism, have exceptional skills in specific areas such as music, art, and numbers. People with savantism are able to perform these skills without lessons or practice	topic_aut
74174	2	355066	5	NULL	NULL	0	NULL	savants	GroupOfPeople		is skilled in		exceptionally			music	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	People with a form of autism, called savantism, have exceptional skills in specific areas such as music, art, and numbers. People with savantism are able to perform these skills without lessons or practice	topic_aut
74175	3	355066	5	NULL	NULL	0	NULL	savants	GroupOfPeople		is skilled in		exceptionally			art	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	People with a form of autism, called savantism, have exceptional skills in specific areas such as music, art, and numbers. People with savantism are able to perform these skills without lessons or practice	topic_aut
74176	4	355066	5	NULL	NULL	0	NULL	savants	GroupOfPeople		is skilled in		exceptionally			numbers	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	People with a form of autism, called savantism, have exceptional skills in specific areas such as music, art, and numbers. People with savantism are able to perform these skills without lessons or practice	topic_aut
75434	1	355068	11	NULL	NULL	0	NULL	Panton-Valentine leukocidin	Chemical		is					PVL	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Panton-Valentine leukocidin (PVL) is a cytotoxin—one of the β-pore-forming toxins. The presence of PVL is associated with increased virulence of certain strains (isolates) of Staphylococcus aureus. 	topic_mrs
75435	2	355068	11	NULL	NULL	NULL	NULL	Panton-Valentine leukocidin	Chemical		is a type of 					 cytotoxin	Chemical	β-pore-forming			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Panton-Valentine leukocidin (PVL) is a cytotoxin—one of the β-pore-forming toxins. The presence of PVL is associated with increased virulence of certain strains (isolates) of Staphylococcus aureus. 	topic_mrs
75436	3	355068	11	NULL	NULL	0	NULL	Panton-Valentine leukocidin	Chemical		increased		may			virulence	PhysicalPhenomenon	Staphylococcus aureus			NULL		0	NULL	NULL	NULL	NULL	NULL	Panton-Valentine leukocidin (PVL) is a cytotoxin—one of the β-pore-forming toxins. The presence of PVL is associated with increased virulence of certain strains (isolates) of Staphylococcus aureus. 	topic_mrs
75437	1	355069	11	NULL	NULL	0	NULL	community-associated Methicillin-resistant Staphylococcus aureus	Organism		is					CA-MRSA	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	It is present in the majority of community-associated Methicillin-resistant Staphylococcus aureus (CA-MRSA) isolates studied and is the cause of necrotic lesions involving the skin or mucosa, including necrotic hemorrhagic pneumonia. 	topic_mrs
75438	2	355069	11	NULL	NULL	0	NULL	community-associated Methicillin-resistant Staphylococcus aureus	Organism		cause					necrotic lesions	Process	skin;;mucosa			NULL		0	NULL	NULL	NULL	NULL	NULL	It is present in the majority of community-associated Methicillin-resistant Staphylococcus aureus (CA-MRSA) isolates studied and is the cause of necrotic lesions involving the skin or mucosa, including necrotic hemorrhagic pneumonia. 	topic_mrs
75439	3	355069	11	NULL	NULL	0	NULL	community-associated Methicillin-resistant Staphylococcus aureus	Organism		cause					necrotic hemorrhagic pneumonia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	It is present in the majority of community-associated Methicillin-resistant Staphylococcus aureus (CA-MRSA) isolates studied and is the cause of necrotic lesions involving the skin or mucosa, including necrotic hemorrhagic pneumonia. 	topic_mrs
76352	1	355070	11	NULL	NULL	0	NULL	Tea tree oil	Chemical		is also known as					melaleuca oil	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Tea tree oil, or melaleuca oil, is a pale yellow colour to nearly clear essential oil with a fresh camphoraceous odor.[	topic_mrs
76353	2	355070	11	NULL	NULL	0	NULL	Tea tree oil	Chemical		colored 					pale yellow	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Tea tree oil, or melaleuca oil, is a pale yellow colour to nearly clear essential oil with a fresh camphoraceous odor.[	topic_mrs
76354	3	355070	11	NULL	NULL	0	NULL	Tea tree oil	Chemical		is a type of 					essential oil 	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Tea tree oil, or melaleuca oil, is a pale yellow colour to nearly clear essential oil with a fresh camphoraceous odor.[	topic_mrs
76355	4	355070	11	NULL	NULL	0	NULL	Tea tree oil	Chemical		has a					fresh camphoraceous odor	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Tea tree oil, or melaleuca oil, is a pale yellow colour to nearly clear essential oil with a fresh camphoraceous odor.[	topic_mrs
75440	1	355071	11	NULL	NULL	0	NULL	Lemongrass oil	Chemical		is a type of 					pesticide	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Lemongrass oil is used as a pesticide and a preservative. Research shows that lemongrass oil has anti-fungal properties	topic_mrs
75441	2	355071	11	NULL	NULL	0	NULL	Lemongrass oil	Chemical		is a type of 					preservative	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Lemongrass oil is used as a pesticide and a preservative. Research shows that lemongrass oil has anti-fungal properties	topic_mrs
75442	3	355071	11	NULL	NULL	NULL	NULL	lemongrass oil 	Chemical		act as					anti-fungal	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Lemongrass oil is used as a pesticide and a preservative. Research shows that lemongrass oil has anti-fungal properties	topic_mrs
76358	1	355073	11	NULL	NULL	0	NULL	Lincosamides	Chemical		are a class of					antibiotics	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Lincosamides (eg. lincomycin, clindamycin) are a class of antibiotics. NULL	topic_mrs
76359	2	355073	11	NULL	NULL	0	NULL	lincomycin	Chemical		is a type of 					Lincosamides	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Lincosamides (eg. lincomycin, clindamycin) are a class of antibiotics. NULL	topic_mrs
76360	3	355073	11	NULL	NULL	0	NULL	clindamycin	Chemical		is a type of 					Lincosamides	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Lincosamides (eg. lincomycin, clindamycin) are a class of antibiotics. NULL	topic_mrs
74177	1	355074	5	NULL	NULL	NULL	NULL	fT	GP		is implicated in					social development	MentalProcess				NULL		NULL	NULL	NULL	NULL	NULL	NULL	fT was also positively correlated with restricted interests in boys. CONCLUSIONS: These findings implicate fT in both social development and attentional focus. They may also have implications for understanding the sex ratio in autism	topic_aut
74178	2	355074	5	NULL	NULL	0	NULL	fT	GP		is implicated in					attentional focus	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	fT was also positively correlated with restricted interests in boys. CONCLUSIONS: These findings implicate fT in both social development and attentional focus. They may also have implications for understanding the sex ratio in autism	topic_aut
74179	3	355074	5	NULL	NULL	0	NULL	fT	GP		is implicated in					autism	MedicalFinding	understanding of;;sex ratio in			NULL		0	NULL	NULL	NULL	NULL	NULL	fT was also positively correlated with restricted interests in boys. CONCLUSIONS: These findings implicate fT in both social development and attentional focus. They may also have implications for understanding the sex ratio in autism	topic_aut
74180	2	355075	5	NULL	NULL	0	NULL	fT	GP		correlates with		positively			statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	fT was also positively correlated with restricted interests in boys. 	topic_aut
74181	1	355075	5	NULL	NULL	NULL	NULL	restricted interests	MentalProcess		is observed in					boys	Organism				NULL		NULL	NULL	NULL	NULL	NULL	NULL	fT was also positively correlated with restricted interests in boys. 	topic_aut
74182	1	355076	5	NULL	NULL	NULL	NULL	ASD children	GroupOfPeople		engage in					rocking	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Many children with ASD engage in repetitive movements such as rocking and twirling, or in self-abusive behavior such as biting or head-banging	topic_aut
74183	2	355076	5	NULL	NULL	0	NULL	ASD children	GroupOfPeople		engage in					twirling	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Many children with ASD engage in repetitive movements such as rocking and twirling, or in self-abusive behavior such as biting or head-banging	topic_aut
74184	3	355076	5	NULL	NULL	0	NULL	rocking	MedicalFinding		is a type of					repetitive movement	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Many children with ASD engage in repetitive movements such as rocking and twirling, or in self-abusive behavior such as biting or head-banging	topic_aut
74185	4	355076	5	NULL	NULL	0	NULL	twirling	MedicalFinding		is a type of					repetitive movement	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Many children with ASD engage in repetitive movements such as rocking and twirling, or in self-abusive behavior such as biting or head-banging	topic_aut
74186	5	355076	5	NULL	NULL	0	NULL	ASD children	GroupOfPeople		engage in					biting	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Many children with ASD engage in repetitive movements such as rocking and twirling, or in self-abusive behavior such as biting or head-banging	topic_aut
74187	6	355076	5	NULL	NULL	0	NULL	ASD children	GroupOfPeople		engage in					head-banging	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Many children with ASD engage in repetitive movements such as rocking and twirling, or in self-abusive behavior such as biting or head-banging	topic_aut
74188	7	355076	5	NULL	NULL	0	NULL	biting	MedicalFinding		is a type of					self-abusive behaviour	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Many children with ASD engage in repetitive movements such as rocking and twirling, or in self-abusive behavior such as biting or head-banging	topic_aut
74189	8	355076	5	NULL	NULL	0	NULL	head-banging	MedicalFinding		is a type of					self-abusive behaviour	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Many children with ASD engage in repetitive movements such as rocking and twirling, or in self-abusive behavior such as biting or head-banging	topic_aut
74190	9	355076	5	NULL	NULL	0	NULL	statement 5	Process		is an alternative to					statement 6	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Many children with ASD engage in repetitive movements such as rocking and twirling, or in self-abusive behavior such as biting or head-banging	topic_aut
74194	1	355078	5	NULL	NULL	0	NULL	ASD children	GroupOfPeople		is at risk of		higher			Fragile X syndrome	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Children with ASD appear to have a higher than normal risk for certain co-occurring conditions, including Fragile X syndrome (which causes mental retardation), tuberous sclerosis (in which tumors grow on the brain), epileptic seizures, Tourette syndrome, learning disabilities, and attention deficit disorder.  About 20 to 30 percent of children with ASD develop epilepsy by the time they reach adulthood	topic_aut
74195	2	355078	5	NULL	NULL	0	NULL	Fragile X syndrome	MedicalFinding		causes					mental retardation	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Children with ASD appear to have a higher than normal risk for certain co-occurring conditions, including Fragile X syndrome (which causes mental retardation), tuberous sclerosis (in which tumors grow on the brain), epileptic seizures, Tourette syndrome, learning disabilities, and attention deficit disorder.  About 20 to 30 percent of children with ASD develop epilepsy by the time they reach adulthood	topic_aut
74196	3	355078	5	NULL	NULL	0	NULL	ASD children	GroupOfPeople		is at risk of		higher			tuberous sclerosis	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Children with ASD appear to have a higher than normal risk for certain co-occurring conditions, including Fragile X syndrome (which causes mental retardation), tuberous sclerosis (in which tumors grow on the brain), epileptic seizures, Tourette syndrome, learning disabilities, and attention deficit disorder.  About 20 to 30 percent of children with ASD develop epilepsy by the time they reach adulthood	topic_aut
74198	4	355078	5	NULL	NULL	0	NULL	tuberous sclerosis	MedicalFinding		causes					tumors	MedicalFinding	growth of			NULL	brain	0	NULL	NULL	NULL	NULL	NULL	Children with ASD appear to have a higher than normal risk for certain co-occurring conditions, including Fragile X syndrome (which causes mental retardation), tuberous sclerosis (in which tumors grow on the brain), epileptic seizures, Tourette syndrome, learning disabilities, and attention deficit disorder.  About 20 to 30 percent of children with ASD develop epilepsy by the time they reach adulthood	topic_aut
74199	5	355078	5	NULL	NULL	0	NULL	ASD children	GroupOfPeople		is at risk of		higher			epileptic seizures	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Children with ASD appear to have a higher than normal risk for certain co-occurring conditions, including Fragile X syndrome (which causes mental retardation), tuberous sclerosis (in which tumors grow on the brain), epileptic seizures, Tourette syndrome, learning disabilities, and attention deficit disorder.  About 20 to 30 percent of children with ASD develop epilepsy by the time they reach adulthood	topic_aut
74200	6	355078	5	NULL	NULL	0	NULL	ASD children	GroupOfPeople		is at risk of		higher			Tourette syndrome	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Children with ASD appear to have a higher than normal risk for certain co-occurring conditions, including Fragile X syndrome (which causes mental retardation), tuberous sclerosis (in which tumors grow on the brain), epileptic seizures, Tourette syndrome, learning disabilities, and attention deficit disorder.  About 20 to 30 percent of children with ASD develop epilepsy by the time they reach adulthood	topic_aut
74201	7	355078	5	NULL	NULL	0	NULL	ASD children	GroupOfPeople		is at risk of		higher			learning disabilities	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Children with ASD appear to have a higher than normal risk for certain co-occurring conditions, including Fragile X syndrome (which causes mental retardation), tuberous sclerosis (in which tumors grow on the brain), epileptic seizures, Tourette syndrome, learning disabilities, and attention deficit disorder.  About 20 to 30 percent of children with ASD develop epilepsy by the time they reach adulthood	topic_aut
74202	8	355078	5	NULL	NULL	0	NULL	ASD children	GroupOfPeople		is at risk of		higher			attention deficit disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Children with ASD appear to have a higher than normal risk for certain co-occurring conditions, including Fragile X syndrome (which causes mental retardation), tuberous sclerosis (in which tumors grow on the brain), epileptic seizures, Tourette syndrome, learning disabilities, and attention deficit disorder.  About 20 to 30 percent of children with ASD develop epilepsy by the time they reach adulthood	topic_aut
74203	9	355078	5	NULL	NULL	0	NULL	ASD children	GroupOfPeople		develops					epilepsy	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Children with ASD appear to have a higher than normal risk for certain co-occurring conditions, including Fragile X syndrome (which causes mental retardation), tuberous sclerosis (in which tumors grow on the brain), epileptic seizures, Tourette syndrome, learning disabilities, and attention deficit disorder.  About 20 to 30 percent of children with ASD develop epilepsy by the time they reach adulthood	topic_aut
74204	10	355078	5	NULL	NULL	0	NULL	statement 9	Process		occurs before					adulthood	Time				NULL		0	NULL	NULL	NULL	NULL	NULL	Children with ASD appear to have a higher than normal risk for certain co-occurring conditions, including Fragile X syndrome (which causes mental retardation), tuberous sclerosis (in which tumors grow on the brain), epileptic seizures, Tourette syndrome, learning disabilities, and attention deficit disorder.  About 20 to 30 percent of children with ASD develop epilepsy by the time they reach adulthood	topic_aut
74206	1	355079	5	NULL	NULL	0	NULL	serotonin	Chemical	abnormal levels of 	is present in					ASD patients	GroupOfPeople	brain of			NULL		0	NULL	NULL	NULL	NULL	NULL	Other studies suggest that people with ASD have abnormal levels of serotonin or other neurotransmitters in the brain	topic_aut
74207	2	355079	5	NULL	NULL	0	NULL	neurotransmitters	Chemical	abnormal levels of	is present in					ASD patients	GroupOfPeople	brain of			NULL		0	NULL	NULL	NULL	NULL	NULL	Other studies suggest that people with ASD have abnormal levels of serotonin or other neurotransmitters in the brain	topic_aut
74208	3	355079	5	NULL	NULL	0	NULL	serotonin	Chemical		is a type of					neurotransmitter	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Other studies suggest that people with ASD have abnormal levels of serotonin or other neurotransmitters in the brain	topic_aut
74209	1	355080	5	NULL	NULL	0	NULL	parental practices	AbstractConcept		not responsible for					ASD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The theory that parental practices are responsible for ASD has long been disproved. 	topic_aut
74210	1	355082	5	NULL	NULL	0	NULL	manic depression	MedicalFinding		is a type of					emotional disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence also suggests that some emotional disorders, such as manic depression, occur more frequently than average in the families of people with ASD.	topic_aut
74211	2	355082	5	NULL	NULL	0	NULL	manic depression	MedicalFinding		occurs in		frequently			ASD people	GroupOfPeople	families of			NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence also suggests that some emotional disorders, such as manic depression, occur more frequently than average in the families of people with ASD.	topic_aut
74212	1	355083	5	NULL	NULL	0	NULL	MET gene	GP		is involved in					brain	OrganismPart	development of			NULL		0	NULL	NULL	NULL	NULL	NULL	They found a single mutation in a gene called MET, which is known to be involved in brain development, regulation of the immune system and repair of the gastrointestinal system. All of these systems can be affected in children with autism.	topic_aut
74213	2	355083	5	NULL	NULL	0	NULL	MET gene	GP		is involved in					immune system	OrganismPart	regulation of			NULL		0	NULL	NULL	NULL	NULL	NULL	They found a single mutation in a gene called MET, which is known to be involved in brain development, regulation of the immune system and repair of the gastrointestinal system. All of these systems can be affected in children with autism.	topic_aut
74215	3	355083	5	NULL	NULL	0	NULL	MET gene	GP		is involved in					gastrointestinal system	OrganismPart	repair of			NULL		0	NULL	NULL	NULL	NULL	NULL	They found a single mutation in a gene called MET, which is known to be involved in brain development, regulation of the immune system and repair of the gastrointestinal system. All of these systems can be affected in children with autism.	topic_aut
74216	4	355083	5	NULL	NULL	0	NULL	brain	OrganismPart		is affected in					autistic children	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	They found a single mutation in a gene called MET, which is known to be involved in brain development, regulation of the immune system and repair of the gastrointestinal system. All of these systems can be affected in children with autism.	topic_aut
74217	5	355083	5	NULL	NULL	0	NULL	immune system	OrganismPart		is affected in					autistic children	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	They found a single mutation in a gene called MET, which is known to be involved in brain development, regulation of the immune system and repair of the gastrointestinal system. All of these systems can be affected in children with autism.	topic_aut
74218	6	355083	5	NULL	NULL	0	NULL	gastrointestinal system	OrganismPart		is affected in					autistic children	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	They found a single mutation in a gene called MET, which is known to be involved in brain development, regulation of the immune system and repair of the gastrointestinal system. All of these systems can be affected in children with autism.	topic_aut
74219	1	355084	5	NULL	NULL	0	NULL	MET	GP		is					Mesenchymal epithelial transition factor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	    MET (Mesenchymal epithelial transition factor), also known as hepatocyte growth factor receptor (HGFR) is a proto-oncogenic receptor tyrosine kinase	topic_aut
74220	2	355084	5	NULL	NULL	0	NULL	HGFR	GP		is					hepatocyte growth factor receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	    MET (Mesenchymal epithelial transition factor), also known as hepatocyte growth factor receptor (HGFR) is a proto-oncogenic receptor tyrosine kinase	topic_aut
74221	3	355084	5	NULL	NULL	0	NULL	MET	GP		is a synonym of					hepatocyte growth factor receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	    MET (Mesenchymal epithelial transition factor), also known as hepatocyte growth factor receptor (HGFR) is a proto-oncogenic receptor tyrosine kinase	topic_aut
74222	4	355084	5	NULL	NULL	0	NULL	MET	GP		is a type of					proto-oncogenic receptor tyrosine kinase	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	    MET (Mesenchymal epithelial transition factor), also known as hepatocyte growth factor receptor (HGFR) is a proto-oncogenic receptor tyrosine kinase	topic_aut
74228	1	355086	5	NULL	NULL	NULL	NULL	television viewing	Process	early childhood	triggers		potentially			autism	MedicalFinding	onset of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	“The analysis shows that early childhood television viewing could be an environmental trigger for the onset of autism and strongly points to the need for more research by experts in the field of autism	topic_aut
74229	1	355087	5	NULL	NULL	0	NULL	autistic children	GroupOfPeople		is prone to					spontaneous mutations	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	It turned out that children with autism were much more likely than other kids to have these 'spontaneous' mutations	topic_aut
74230	2	355087	5	NULL	NULL	0	NULL	normal children	GroupOfPeople		is prone to					spontaneous mutations	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	It turned out that children with autism were much more likely than other kids to have these 'spontaneous' mutations	topic_aut
74231	3	355087	5	NULL	NULL	0	NULL	statement 1	Process		is more likely than					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	It turned out that children with autism were much more likely than other kids to have these 'spontaneous' mutations	topic_aut
74232	1	355088	5	NULL	NULL	0	NULL	oxytocin	GP		is a type of					hormone	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	For example, Sebat says one child in the study was missing a copy of the gene for oxytocin – a hormone that seems to influence social behavior.	topic_aut
74233	2	355088	5	NULL	NULL	0	NULL	oxytocin gene	GP		influence					social behavior	AbstractConcept				NULL		0	NULL	NULL	NULL	NULL	NULL	For example, Sebat says one child in the study was missing a copy of the gene for oxytocin – a hormone that seems to influence social behavior.	topic_aut
74234	1	355091	5	NULL	NULL	0	NULL	chromosome 16	Chromosome	variation of	is present in					autistic people	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	On Thursday, scientists reported that 1 percent of people with autism share a variation on chromosome 16	topic_aut
74235	1	355093	5	NULL	NULL	0	NULL	CNVs	Chromosome		over-represented in		heavily			autistic people	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	In the article the group reveals that a survey of 1,000 individuals with autism and 1,300 without showed that Copy Number Variants (CNVs) - sub-microscopic abnormalities in the chromosomes - are heavily over-represented in autistic people	topic_aut
74236	2	355093	5	NULL	NULL	0	NULL	CNVs	Chromosome		is					Copy Number Variants	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	In the article the group reveals that a survey of 1,000 individuals with autism and 1,300 without showed that Copy Number Variants (CNVs) - sub-microscopic abnormalities in the chromosomes - are heavily over-represented in autistic people	topic_aut
74237	3	355093	5	NULL	NULL	0	NULL	chromosomes	Chromosome	sub-microscopic abnormalities of	is known as					Copy Number Variants	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	In the article the group reveals that a survey of 1,000 individuals with autism and 1,300 without showed that Copy Number Variants (CNVs) - sub-microscopic abnormalities in the chromosomes - are heavily over-represented in autistic people	topic_aut
75443	1	355095	11	NULL	NULL	0	NULL	Linezolid	Chemical		is a type of 					synthetic antibiotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Linezolid is a synthetic antibiotic used for the treatment of serious infections caused by Gram-positive bacteria that are resistant to several other antibiotics	topic_mrs
75444	2	355095	11	NULL	NULL	0	NULL	Gram-positive bacteria	Organism		cause					infections	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Linezolid is a synthetic antibiotic used for the treatment of serious infections caused by Gram-positive bacteria that are resistant to several other antibiotics	topic_mrs
75445	3	355095	11	NULL	NULL	0	NULL	Linezolid	Chemical		treats					statement 2					NULL		0	NULL	NULL	NULL	NULL	NULL	Linezolid is a synthetic antibiotic used for the treatment of serious infections caused by Gram-positive bacteria that are resistant to several other antibiotics	topic_mrs
75446	1	355096	11	NULL	NULL	0	NULL	S. aureus	Organism		colonizes					anterior nares	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	S. aureus most commonly colonizes the anterior nares (the nostrils), although the rest of the respiratory tract, opened wounds, intravenous catheters, and urinary tract are also potential sites for infection. Healthy individuals may carry MRSA asymptomatically for periods ranging from a few weeks to many years.	topic_mrs
75447	2	355096	11	NULL	NULL	0	NULL	anterior nares	OrganismPart		is					nostrils	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	S. aureus most commonly colonizes the anterior nares (the nostrils), although the rest of the respiratory tract, opened wounds, intravenous catheters, and urinary tract are also potential sites for infection. Healthy individuals may carry MRSA asymptomatically for periods ranging from a few weeks to many years.	topic_mrs
75448	3	355096	11	NULL	NULL	NULL	NULL	S. aureus	OrganismPart		infects					respiratory tract	OrganismPart				NULL		NULL	NULL	NULL	NULL	NULL	NULL	S. aureus most commonly colonizes the anterior nares (the nostrils), although the rest of the respiratory tract, opened wounds, intravenous catheters, and urinary tract are also potential sites for infection. Healthy individuals may carry MRSA asymptomatically for periods ranging from a few weeks to many years.	topic_mrs
75449	4	355096	11	NULL	NULL	NULL	NULL	S. aureus	Organism		infects					opened wounds	OrganismPart				NULL		NULL	NULL	NULL	NULL	NULL	NULL	S. aureus most commonly colonizes the anterior nares (the nostrils), although the rest of the respiratory tract, opened wounds, intravenous catheters, and urinary tract are also potential sites for infection. Healthy individuals may carry MRSA asymptomatically for periods ranging from a few weeks to many years.	topic_mrs
75450	5	355096	11	NULL	NULL	NULL	NULL	S. aureus	Organism		infects					intravenous catheters	MedicalProcedure				NULL		NULL	NULL	NULL	NULL	NULL	NULL	S. aureus most commonly colonizes the anterior nares (the nostrils), although the rest of the respiratory tract, opened wounds, intravenous catheters, and urinary tract are also potential sites for infection. Healthy individuals may carry MRSA asymptomatically for periods ranging from a few weeks to many years.	topic_mrs
75451	6	355096	11	NULL	NULL	NULL	NULL	S. aureus	Organism		infects					urinary tract	OrganismPart				NULL		NULL	NULL	NULL	NULL	NULL	NULL	S. aureus most commonly colonizes the anterior nares (the nostrils), although the rest of the respiratory tract, opened wounds, intravenous catheters, and urinary tract are also potential sites for infection. Healthy individuals may carry MRSA asymptomatically for periods ranging from a few weeks to many years.	topic_mrs
75452	7	355096	11	NULL	NULL	0	NULL	MRSA	Organism		colonizes		may			asymptomatically	Process	in Healthy individuals			NULL		0	NULL	NULL	NULL	NULL	NULL	S. aureus most commonly colonizes the anterior nares (the nostrils), although the rest of the respiratory tract, opened wounds, intravenous catheters, and urinary tract are also potential sites for infection. Healthy individuals may carry MRSA asymptomatically for periods ranging from a few weeks to many years.	topic_mrs
75453	1	355097	11	NULL	NULL	0	NULL	MRSA	Organism		progress to		may			topical symptoms	Process	initial			NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA may progress substantially within 24–48 hours of initial topical symptoms. After 72 hours MRSA can take hold in human tissues and eventually become resistant to treatment. The initial presentation of MRSA is small red bumps that resemble pimples, spider bites, or boils that may be accompanied by fever and occasionally rashes. 	topic_mrs
75454	2	355097	11	NULL	NULL	0	NULL	MRSA	Organism		presents					small red bumps	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA may progress substantially within 24–48 hours of initial topical symptoms. After 72 hours MRSA can take hold in human tissues and eventually become resistant to treatment. The initial presentation of MRSA is small red bumps that resemble pimples, spider bites, or boils that may be accompanied by fever and occasionally rashes. 	topic_mrs
75455	3	355097	11	NULL	NULL	0	NULL	statement 2	Process		accompanies					fever	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA may progress substantially within 24–48 hours of initial topical symptoms. After 72 hours MRSA can take hold in human tissues and eventually become resistant to treatment. The initial presentation of MRSA is small red bumps that resemble pimples, spider bites, or boils that may be accompanied by fever and occasionally rashes. 	topic_mrs
75456	4	355097	11	NULL	NULL	0	NULL	statement 2	Process		accompanies					 rashes	Process	occasionally			NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA may progress substantially within 24–48 hours of initial topical symptoms. After 72 hours MRSA can take hold in human tissues and eventually become resistant to treatment. The initial presentation of MRSA is small red bumps that resemble pimples, spider bites, or boils that may be accompanied by fever and occasionally rashes. 	topic_mrs
75457	1	355098	11	NULL	NULL	0	NULL	Gram-positive organism	Organism		causes					infections	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Daptomycin is a novel lipopeptide antibiotic used in the treatment of certain infections caused by Gram-positive organisms. 	topic_mrs
75458	2	355098	11	NULL	NULL	0	NULL	Daptomycin	Chemical		is a type of 					lipopeptide antibiotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Daptomycin is a novel lipopeptide antibiotic used in the treatment of certain infections caused by Gram-positive organisms. 	topic_mrs
75459	3	355098	11	NULL	NULL	0	NULL	Daptomycin	Chemical		treats					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Daptomycin is a novel lipopeptide antibiotic used in the treatment of certain infections caused by Gram-positive organisms. 	topic_mrs
76361	1	355099	11	NULL	NULL	0	NULL	lipopeptide	Chemical		 consisting of					lipid	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	A lipopeptide is a molecule consisting of a lipid connected to a peptide. Certain lipopeptides are used as antibiotics.	topic_mrs
76362	2	355099	11	NULL	NULL	0	NULL	lipopeptide	Chemical		consisting of					peptide	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	A lipopeptide is a molecule consisting of a lipid connected to a peptide. Certain lipopeptides are used as antibiotics.	topic_mrs
76363	3	355099	11	NULL	NULL	0	NULL	statement 1	Chemical		connected to 					statement 2	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	A lipopeptide is a molecule consisting of a lipid connected to a peptide. Certain lipopeptides are used as antibiotics.	topic_mrs
76364	4	355099	11	NULL	NULL	0	NULL	lipopeptides	Chemical	Certain	are used as					antibiotics	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	A lipopeptide is a molecule consisting of a lipid connected to a peptide. Certain lipopeptides are used as antibiotics.	topic_mrs
75460	1	355100	11	NULL	NULL	NULL	NULL	bone	Organism part	infection of	is known as					Osteomyelitis	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Osteomyelitis simply means an infection of the bone or bone marrow.	topic_mrs
76622	2	355100	11	NULL	NULL	0	NULL	bone marrow	Organism part	infection of	is known as					osteomyelitis	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Osteomyelitis simply means an infection of the bone or bone marrow.	topic_mrs
75575	1	355101	7	NULL	NULL	NULL	NULL	bipolar II/hypomania	MedicalFinding	rapid cycling	 increased risk in					Women	GroupOfPeople				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Most studies, but not all, report an almost equal gender ratio in the prevalence of bipolar disorder but the majority of studies do report an increased risk in women of bipolar II/hypomania, rapid cycling and mixed episodes.	topic_bd
75576	2	355101	7	NULL	NULL	NULL	NULL	bipolar II/hypomania	MedicalFinding	mixed episodes of	increased risk in					Women	GroupOfPeople				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Most studies, but not all, report an almost equal gender ratio in the prevalence of bipolar disorder but the majority of studies do report an increased risk in women of bipolar II/hypomania, rapid cycling and mixed episodes.	topic_bd
75577	1	355102	7	NULL	NULL	0	NULL	bipolar disorder	MedicalFinding		impacts					reproductive life events	MedicalFinding				NULL	Women	0	NULL	NULL	NULL	NULL	NULL	Unsurprisingly, however, perhaps the major distinction between men and women with bipolar disorder is the impact that reproductive life events, particularly childbirth, have on women with this diagnosis.	topic_bd
75578	1	355109	7	NULL	NULL	0	NULL	Geodon	Chemical		is a type of					antipsychotic medication	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Geodon (ziprasidone) is an antipsychotic medication. 	topic_bd
75579	2	355109	7	NULL	NULL	0	NULL	Geodon 	Chemical		is					ziprasidone	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Geodon (ziprasidone) is an antipsychotic medication. 	topic_bd
75580	1	355110	7	NULL	NULL	NULL	NULL	Geodon	Chemical		is used to treat					schizophrenia	MedicalFinding				NULL	adults	NULL	NULL	NULL	NULL	NULL	NULL	Geodon is used to treat schizophrenia and the manic symptoms of bipolar disorder (manic depression) in adults and children who are at least 10 years old.	topic_bd
75581	2	355110	7	NULL	NULL	0	NULL	Geodon	Chemical		is used to treat					bipolar disorder	MedicalFinding	manic symptoms of			NULL	adults	0	NULL	NULL	NULL	NULL	NULL	Geodon is used to treat schizophrenia and the manic symptoms of bipolar disorder (manic depression) in adults and children who are at least 10 years old.	topic_bd
75582	3	355110	7	NULL	NULL	NULL	NULL	Geodon	Chemical		is used to treat					schizophrenia	MedicalFinding				NULL	children	NULL	NULL	NULL	NULL	NULL	NULL	Geodon is used to treat schizophrenia and the manic symptoms of bipolar disorder (manic depression) in adults and children who are at least 10 years old.	topic_bd
75583	4	355110	7	NULL	NULL	NULL	NULL	Geodon	Chemical		is used to treat					bipolar disorder	MedicalFinding	manic symptoms of			NULL	children	NULL	NULL	NULL	NULL	NULL	NULL	Geodon is used to treat schizophrenia and the manic symptoms of bipolar disorder (manic depression) in adults and children who are at least 10 years old.	topic_bd
75584	5	355110	7	NULL	NULL	0	NULL	bipolar disorder	MedicalFinding		is a type of					manic depression	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Geodon is used to treat schizophrenia and the manic symptoms of bipolar disorder (manic depression) in adults and children who are at least 10 years old.	topic_bd
75585	1	355111	7	NULL	NULL	0	NULL	dysphoria	MedicalFinding		is a state of					feeling unhappy	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	dysphoria is actually very straightforward - a state of feeling unwell or unhappy.	topic_bd
75586	2	355111	7	NULL	NULL	0	NULL	dysphoria	MedicalFinding		is a state of					feeling unwell	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	dysphoria is actually very straightforward - a state of feeling unwell or unhappy.	topic_bd
75587	3	355111	7	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	dysphoria is actually very straightforward - a state of feeling unwell or unhappy.	topic_bd
75588	1	355112	7	NULL	NULL	0	NULL	Dysphoric depression	MedicalFinding		is a type of					mixed episode	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Dysphoric depression, which many people think of as a mixed episode, consists of "intrusions of hypomanic symptoms or hyperthymic traits into a retarded major depressive episode" (Merck). 	topic_bd
75589	2	355112	7	NULL	NULL	0	NULL	Dysphoric depression	MedicalFinding		consist of					hypomanic symptoms	MedicalFinding	intrusions of			NULL		0	NULL	NULL	NULL	NULL	NULL	Dysphoric depression, which many people think of as a mixed episode, consists of "intrusions of hypomanic symptoms or hyperthymic traits into a retarded major depressive episode" (Merck). 	topic_bd
75590	3	355112	7	NULL	NULL	0	NULL	Dysphoric depression	MedicalFinding		consist of					retarded major depressive episode	MedicalFinding	hyperthymic traits into 			NULL		0	NULL	NULL	NULL	NULL	NULL	Dysphoric depression, which many people think of as a mixed episode, consists of "intrusions of hypomanic symptoms or hyperthymic traits into a retarded major depressive episode" (Merck). 	topic_bd
75591	1	355115	7	NULL	NULL	0	NULL	Lithium	Chemical		cause					Thyroid Goiters	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	You need to know that Lithium can cause Thyroid Goiters. 	topic_bd
75592	1	355116	7	NULL	NULL	0	NULL	BP'ers	GroupOfPeople		have					trauma issues	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Since many BP'ers have trauma issues EDMR is helpful for resolving trauma and another common type is Dialectal Behavior Therapy.	topic_bd
75593	2	355116	7	NULL	NULL	0	NULL	EDMR	MedicalProcedure		is helpful for					trauma	MedicalFinding	resolving			NULL		0	NULL	NULL	NULL	NULL	NULL	Since many BP'ers have trauma issues EDMR is helpful for resolving trauma and another common type is Dialectal Behavior Therapy.	topic_bd
75594	3	355116	7	NULL	NULL	0	NULL	Dialectal Behavior Therapy	MedicalProcedure		is helpful for					trauma	MedicalFinding	resolving			NULL		0	NULL	NULL	NULL	NULL	NULL	Since many BP'ers have trauma issues EDMR is helpful for resolving trauma and another common type is Dialectal Behavior Therapy.	topic_bd
74238	1	355117	5	NULL	NULL	NULL	NULL	 D(2) receptor (D(2)R)	GP		is a subtype of					dopamine receptor	GP				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Among the characterized dopamine receptor subtypes, D(2) receptor (D(2)R) and D(3) receptor (D(3)R) are the main targets of neuroleptics that are currently in use. In particular, D(3)R is closely related to the etiology of schizophrenia and drug addiction. 	topic_sch
74240	2	355117	5	NULL	NULL	0	NULL	D(3) receptor (D(3)R)	GP		is a subtype of					dopamine receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Among the characterized dopamine receptor subtypes, D(2) receptor (D(2)R) and D(3) receptor (D(3)R) are the main targets of neuroleptics that are currently in use. In particular, D(3)R is closely related to the etiology of schizophrenia and drug addiction. 	topic_sch
74241	3	355117	5	NULL	NULL	0	NULL	D(2) receptor (D(2)R)	GP		is a target of		main			neuroleptics	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Among the characterized dopamine receptor subtypes, D(2) receptor (D(2)R) and D(3) receptor (D(3)R) are the main targets of neuroleptics that are currently in use. In particular, D(3)R is closely related to the etiology of schizophrenia and drug addiction. 	topic_sch
74242	4	355117	5	NULL	NULL	0	NULL	D(3) receptor (D(3)R)	GP		is a target of		main			neuroleptics	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Among the characterized dopamine receptor subtypes, D(2) receptor (D(2)R) and D(3) receptor (D(3)R) are the main targets of neuroleptics that are currently in use. In particular, D(3)R is closely related to the etiology of schizophrenia and drug addiction. 	topic_sch
74243	5	355117	5	NULL	NULL	NULL	NULL	 D(3)R	GP		is related to		closely			schizophrenia	MedicalFinding	etiology of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Among the characterized dopamine receptor subtypes, D(2) receptor (D(2)R) and D(3) receptor (D(3)R) are the main targets of neuroleptics that are currently in use. In particular, D(3)R is closely related to the etiology of schizophrenia and drug addiction. 	topic_sch
74244	6	355117	5	NULL	NULL	NULL	NULL	 D(3)R	GP		is related to		closely			drug addiction	MentalProcess	etiology of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Among the characterized dopamine receptor subtypes, D(2) receptor (D(2)R) and D(3) receptor (D(3)R) are the main targets of neuroleptics that are currently in use. In particular, D(3)R is closely related to the etiology of schizophrenia and drug addiction. 	topic_sch
74245	1	355118	5	NULL	NULL	0	NULL	Clozapine	Chemical		delays					treatment resistant schizophrenia patients	GroupOfPeople	hospitalization of			NULL		0	NULL	NULL	NULL	NULL	NULL	Clozapine delays hospitalization in patients with treatment resistant schizophrenia if they are started on clozapine in the community or successfully discharged from hospital following their index admission.	topic_sch
74246	1	355119	5	NULL	NULL	0	NULL	Risperidone	Chemical		is a type of					antipsychotics	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrated that antipsychotic treatment with Risperidone, Olanzapine or Aripiprazole in adolescents affected by Schizophrenia led to significant improvements in symptomatology.	topic_sch
74247	2	355119	5	NULL	NULL	0	NULL	Olanzapine	Chemical		is a type of					antipsychotics	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrated that antipsychotic treatment with Risperidone, Olanzapine or Aripiprazole in adolescents affected by Schizophrenia led to significant improvements in symptomatology.	topic_sch
74248	3	355119	5	NULL	NULL	0	NULL	Aripiprazole	Chemical		is a type of					antipsychotics	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrated that antipsychotic treatment with Risperidone, Olanzapine or Aripiprazole in adolescents affected by Schizophrenia led to significant improvements in symptomatology.	topic_sch
74249	5	355119	5	NULL	NULL	0	NULL	Risperidone	Chemical	treatment	leads to					statement 4	Process	significant improvements in;;symptomatology of			NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrated that antipsychotic treatment with Risperidone, Olanzapine or Aripiprazole in adolescents affected by Schizophrenia led to significant improvements in symptomatology.	topic_sch
74250	4	355119	5	NULL	NULL	0	NULL	adolescents	GroupOfPeople		is affected by					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrated that antipsychotic treatment with Risperidone, Olanzapine or Aripiprazole in adolescents affected by Schizophrenia led to significant improvements in symptomatology.	topic_sch
74251	6	355119	5	NULL	NULL	0	NULL	Olanzapine	Chemical	treatment	leads to					statement 4	Process	significant improvements in;;symptomatology of			NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrated that antipsychotic treatment with Risperidone, Olanzapine or Aripiprazole in adolescents affected by Schizophrenia led to significant improvements in symptomatology.	topic_sch
74252	7	355119	5	NULL	NULL	0	NULL	Aripiprazole	Chemical	treatment	leads to					statement 4	Process	significant improvements in;;symptomatology of			NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrated that antipsychotic treatment with Risperidone, Olanzapine or Aripiprazole in adolescents affected by Schizophrenia led to significant improvements in symptomatology.	topic_sch
74253	1	355120	5	NULL	NULL	0	NULL	schizophrenia people	GroupOfPeople		is at risk of					death	AbstractConcept	premature			NULL		0	NULL	NULL	NULL	NULL	NULL	People with schizophrenia show a two to threefold increased risk to die prematurely than those without schizophrenia. 	topic_sch
74254	2	355120	5	NULL	NULL	0	NULL	non-schizophrenia people	GroupOfPeople		is at risk of					death	AbstractConcept	premature			NULL		0	NULL	NULL	NULL	NULL	NULL	People with schizophrenia show a two to threefold increased risk to die prematurely than those without schizophrenia. 	topic_sch
74255	3	355120	5	NULL	NULL	0	NULL	statement 1	Process		is more likely than					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	People with schizophrenia show a two to threefold increased risk to die prematurely than those without schizophrenia. 	topic_sch
74256	1	355121	5	NULL	NULL	0	NULL	cardiac arrhythmia	MedicalFinding		plays a role in		potentially			schizophrenic patients	GroupOfPeople	sudden death of			NULL		0	NULL	NULL	NULL	NULL	NULL	The exact pathophysiological cause of sudden death in schizophrenia is unknown, but it is likely that cardiac arrhythmia and respiratory abnormalities play potential role.	topic_sch
74257	2	355121	5	NULL	NULL	0	NULL	respiratory abnormalities	MedicalFinding		plays a role in		potentially			schizophrenic patients	GroupOfPeople	sudden death of			NULL		0	NULL	NULL	NULL	NULL	NULL	The exact pathophysiological cause of sudden death in schizophrenia is unknown, but it is likely that cardiac arrhythmia and respiratory abnormalities play potential role.	topic_sch
74316	1	355122	5	NULL	NULL	0	NULL	hyperthyroidism	MedicalFinding	subclinical	is linked to					cardiovascular disease	MedicalFinding	increased risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	As subclinical hyperthyroidism has been linked with increased risk of cardiovascular disease and cerebella progressive atrophy has been observed in patients with schizophrenia, we propose in this paper that subclinical thyroid dysfunction and cerebella volume loss could be considered as new risk factor for sudden cardiac death in schizophrenia.	topic_sch
74317	2	355122	5	NULL	NULL	0	NULL	cerebella progressive atrophy	MedicalFinding		is observed in					schizophrenia patients	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	As subclinical hyperthyroidism has been linked with increased risk of cardiovascular disease and cerebella progressive atrophy has been observed in patients with schizophrenia, we propose in this paper that subclinical thyroid dysfunction and cerebella volume loss could be considered as new risk factor for sudden cardiac death in schizophrenia.	topic_sch
74318	3	355122	5	NULL	NULL	0	NULL	cardiac death	AbstractConcept	sudden	is observed in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	As subclinical hyperthyroidism has been linked with increased risk of cardiovascular disease and cerebella progressive atrophy has been observed in patients with schizophrenia, we propose in this paper that subclinical thyroid dysfunction and cerebella volume loss could be considered as new risk factor for sudden cardiac death in schizophrenia.	topic_sch
74319	4	355122	5	NULL	NULL	0	NULL	thyroid dysfunction	MedicalFinding	subclinical	is a risk factor for		possibly			statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	As subclinical hyperthyroidism has been linked with increased risk of cardiovascular disease and cerebella progressive atrophy has been observed in patients with schizophrenia, we propose in this paper that subclinical thyroid dysfunction and cerebella volume loss could be considered as new risk factor for sudden cardiac death in schizophrenia.	topic_sch
74320	5	355122	5	NULL	NULL	0	NULL	cerebella volume loss	MedicalFinding		is a risk factor for		possibly			statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	As subclinical hyperthyroidism has been linked with increased risk of cardiovascular disease and cerebella progressive atrophy has been observed in patients with schizophrenia, we propose in this paper that subclinical thyroid dysfunction and cerebella volume loss could be considered as new risk factor for sudden cardiac death in schizophrenia.	topic_sch
74258	1	355123	5	NULL	NULL	0	NULL	ADNP/ADNP2	GP	imbalance of;;expression of	impacts		may			schizophrenia	MedicalFinding	progression of			NULL		0	NULL	NULL	NULL	NULL	NULL	Imbalance in ADNP/ADNP2 expression in the schizophrenia brain may impact disease progression.	topic_sch
74259	1	355124	5	NULL	NULL	0	NULL	Akt1 isoform	GP		regulates					hippocampus	OrganismPart	 neuroplasticity of			NULL		0	NULL	NULL	NULL	NULL	NULL	Taken together, these results implicate the Akt1 isoform in regulating hippocampal neuroplasticity and cognition and in contributing to the etiology of schizophrenia.	topic_sch
74260	2	355124	5	NULL	NULL	0	NULL	Akt1 isoform	GP		regulates					cognition	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Taken together, these results implicate the Akt1 isoform in regulating hippocampal neuroplasticity and cognition and in contributing to the etiology of schizophrenia.	topic_sch
74261	3	355124	5	NULL	NULL	0	NULL	Akt1 isoform	GP		contribute to					schizophrenia	MedicalFinding	etiology of			NULL		0	NULL	NULL	NULL	NULL	NULL	Taken together, these results implicate the Akt1 isoform in regulating hippocampal neuroplasticity and cognition and in contributing to the etiology of schizophrenia.	topic_sch
74262	1	355126	5	NULL	NULL	0	NULL	drugs	Chemical	novel	counteracts					schizophrenia	MedicalFinding	cognitive deficits of 			NULL		0	NULL	NULL	NULL	NULL	NULL	This supports the proposal that suppression in GLU release might be a target for the development of novel drugs aimed at counteracting some aspects of cognitive deficits of schizophrenia.	topic_sch
74263	2	355126	5	NULL	NULL	0	NULL	GLU	GP	suppression of;;release of	is a target for		might be			statement 1	Process	development of			NULL		0	NULL	NULL	NULL	NULL	NULL	This supports the proposal that suppression in GLU release might be a target for the development of novel drugs aimed at counteracting some aspects of cognitive deficits of schizophrenia.	topic_sch
74264	1	355127	5	NULL	NULL	0	NULL	SLC6A3 A1343G polymorphism	AbstractConcept		is associated with					SCZ phenotype	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	NULL	NULL	Thus the SLC6A3 A1343G polymorphism was associated to the SCZ phenotype in the investigated sample.	topic_sch
74265	1	355128	5	NULL	NULL	0	NULL	depression	MedicalFinding		is associated with		significantly			schizophrenic persons	GroupOfPeople	nonadherence of			NULL		0	NULL	NULL	NULL	NULL	NULL	Depression and social support deficits were significantly associated with nonadherence in persons with schizophrenia.	topic_sch
74266	2	355128	5	NULL	NULL	0	NULL	social support	AbstractConcept	deficits of	is associated with		significantly			schizophrenic persons	GroupOfPeople	nonadherence of			NULL		0	NULL	NULL	NULL	NULL	NULL	Depression and social support deficits were significantly associated with nonadherence in persons with schizophrenia.	topic_sch
74267	1	355129	5	NULL	NULL	0	NULL	eye gaze	AbstractConcept	deficits of	occurs during					negative social interactions	AbstractConcept				NULL		0	NULL	NULL	NULL	NULL	NULL	Deficits in eye gaze during negative social interactions in patients with schizophrenia.	topic_sch
74268	2	355129	5	NULL	NULL	0	NULL	statement 1	Process		occurs in					schizophrenic patients	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Deficits in eye gaze during negative social interactions in patients with schizophrenia.	topic_sch
74269	1	355130	5	NULL	NULL	0	NULL	Gsk-3	GP	altered activity of	is implicated in					diabetes	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Underscoring their biological significance, altered Gsk-3 activity has been implicated in diabetes, Alzheimers disease, schizophrenia, and bipolar disorder.	topic_sch
74270	2	355130	5	NULL	NULL	0	NULL	Gsk-3	GP	altered activity of	is implicated in					Alzheimers disease	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Underscoring their biological significance, altered Gsk-3 activity has been implicated in diabetes, Alzheimers disease, schizophrenia, and bipolar disorder.	topic_sch
74271	3	355130	5	NULL	NULL	0	NULL	Gsk-3	GP	altered activity of	is implicated in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Underscoring their biological significance, altered Gsk-3 activity has been implicated in diabetes, Alzheimers disease, schizophrenia, and bipolar disorder.	topic_sch
74272	4	355130	5	NULL	NULL	0	NULL	Gsk-3	GP	altered activity of	is implicated in					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Underscoring their biological significance, altered Gsk-3 activity has been implicated in diabetes, Alzheimers disease, schizophrenia, and bipolar disorder.	topic_sch
76365	1	355133	11	NULL	NULL	0	NULL	community-associated MRSA	Organism		causes					 infections	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Most infections caused by these community-associated (CA) MRSA appear to involve the skin	topic_mrs
76366	2	355133	11	NULL	NULL	0	NULL	statement 1	Process		involves					skin	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Most infections caused by these community-associated (CA) MRSA appear to involve the skin	topic_mrs
76367	1	355136	11	NULL	NULL	0	NULL	Alcohol	Chemical		is a type of 					surface sanitizer	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	alcohol-based hand sanitizers were placed in involved areas, Alcohol has been proven to be an effective surface sanitizer against MRSA	topic_mrs
76368	2	355136	11	NULL	NULL	0	NULL	Alcohol	Chemical		is effective against					MRSA	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	alcohol-based hand sanitizers were placed in involved areas, Alcohol has been proven to be an effective surface sanitizer against MRSA	topic_mrs
76369	1	355138	11	NULL	NULL	0	NULL	 MRSA	Organism		is a type of 					bacterium	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	These new evolutions of the MRSA bacterium have been dubbed Vancomycin intermediate-resistant Staphylococcus aureus (VISA).	topic_mrs
76370	2	355138	11	NULL	NULL	0	NULL	MRSA bacterium	Organism		is also known as					Vancomycin intermediate-resistant Staphylococcus aureus 	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	These new evolutions of the MRSA bacterium have been dubbed Vancomycin intermediate-resistant Staphylococcus aureus (VISA).	topic_mrs
76371	3	355138	11	NULL	NULL	0	NULL	Vancomycin intermediate-resistant Staphylococcus aureus 	Organism		is					VISA	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	These new evolutions of the MRSA bacterium have been dubbed Vancomycin intermediate-resistant Staphylococcus aureus (VISA).	topic_mrs
76372	1	355139	11	NULL	NULL	NULL	NULL	Staphylococcus aureus	Organism		cause					staph infections	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Staphylococcus aureus is a facultatively anaerobic, Gram-positive coccus and is the most common cause of staph infections. It is frequently part of the skin flora found in the nose and on skin. About 20% of the human population are long-term carriers of S. aureus.	topic_mrs
76373	2	355139	11	NULL	NULL	0	NULL	Staphylococcus aureus	Organism		is a part of					 skin flora	Organism	nose ;; skin			NULL		0	NULL	NULL	NULL	NULL	NULL	Staphylococcus aureus is a facultatively anaerobic, Gram-positive coccus and is the most common cause of staph infections. It is frequently part of the skin flora found in the nose and on skin. About 20% of the human population are long-term carriers of S. aureus.	topic_mrs
75595	1	355141	7	NULL	NULL	0	NULL	Seroquel	Chemical		is a type of					antipsychotic medication	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Seroquel (quetiapine) is an antipsychotic medication.	topic_bd
75596	2	355141	7	NULL	NULL	0	NULL	Seroquel	Chemical		is					quetiapine	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Seroquel (quetiapine) is an antipsychotic medication.	topic_bd
75597	1	355142	7	NULL	NULL	NULL	NULL	quetiapine	Chemical		inhibits					brain nerves	Process	communication between			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although the mechanism of action of quetiapine is unknown, like other anti-psychotics, it inhibits communication between nerves of the brain. It does this by blocking receptors on the nerves for several neurotransmitters, the chemicals that nerves use to communicate with each other. It is thought that its beneficial effect is due to blocking of the dopamine type 2 (D2) and serotonin type 2 (5-HT2) receptors. 	topic_bd
75598	2	355142	7	NULL	NULL	0	NULL	statement 1	Process		occur by					neurotransmitters	Chemical	blocking receptors of			NULL	nerves	0	NULL	NULL	NULL	NULL	NULL	Although the mechanism of action of quetiapine is unknown, like other anti-psychotics, it inhibits communication between nerves of the brain. It does this by blocking receptors on the nerves for several neurotransmitters, the chemicals that nerves use to communicate with each other. It is thought that its beneficial effect is due to blocking of the dopamine type 2 (D2) and serotonin type 2 (5-HT2) receptors. 	topic_bd
75599	3	355142	7	NULL	NULL	0	NULL	neurotransmitters	Chemical		helps in					nerves	OrganismPart	communication between			NULL		0	NULL	NULL	NULL	NULL	NULL	Although the mechanism of action of quetiapine is unknown, like other anti-psychotics, it inhibits communication between nerves of the brain. It does this by blocking receptors on the nerves for several neurotransmitters, the chemicals that nerves use to communicate with each other. It is thought that its beneficial effect is due to blocking of the dopamine type 2 (D2) and serotonin type 2 (5-HT2) receptors. 	topic_bd
75600	4	355142	7	NULL	NULL	0	NULL	quetiapine	Chemical		blocks					D2 receptors	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Although the mechanism of action of quetiapine is unknown, like other anti-psychotics, it inhibits communication between nerves of the brain. It does this by blocking receptors on the nerves for several neurotransmitters, the chemicals that nerves use to communicate with each other. It is thought that its beneficial effect is due to blocking of the dopamine type 2 (D2) and serotonin type 2 (5-HT2) receptors. 	topic_bd
75601	5	355142	7	NULL	NULL	0	NULL	quetiapine	Chemical		blocks					5-HT2 receptor	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Although the mechanism of action of quetiapine is unknown, like other anti-psychotics, it inhibits communication between nerves of the brain. It does this by blocking receptors on the nerves for several neurotransmitters, the chemicals that nerves use to communicate with each other. It is thought that its beneficial effect is due to blocking of the dopamine type 2 (D2) and serotonin type 2 (5-HT2) receptors. 	topic_bd
75602	6	355142	7	NULL	NULL	0	NULL	D2 receptor	GP		is					dopamine type 2 receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Although the mechanism of action of quetiapine is unknown, like other anti-psychotics, it inhibits communication between nerves of the brain. It does this by blocking receptors on the nerves for several neurotransmitters, the chemicals that nerves use to communicate with each other. It is thought that its beneficial effect is due to blocking of the dopamine type 2 (D2) and serotonin type 2 (5-HT2) receptors. 	topic_bd
75603	7	355142	7	NULL	NULL	NULL	NULL	5-HT2 receptor	GP		is					serotonin type 2 receptor	GP				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although the mechanism of action of quetiapine is unknown, like other anti-psychotics, it inhibits communication between nerves of the brain. It does this by blocking receptors on the nerves for several neurotransmitters, the chemicals that nerves use to communicate with each other. It is thought that its beneficial effect is due to blocking of the dopamine type 2 (D2) and serotonin type 2 (5-HT2) receptors. 	topic_bd
75604	8	355142	7	NULL	NULL	0	NULL	quetiapine	Chemical	beneficial effect of	is due to					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Although the mechanism of action of quetiapine is unknown, like other anti-psychotics, it inhibits communication between nerves of the brain. It does this by blocking receptors on the nerves for several neurotransmitters, the chemicals that nerves use to communicate with each other. It is thought that its beneficial effect is due to blocking of the dopamine type 2 (D2) and serotonin type 2 (5-HT2) receptors. 	topic_bd
75605	9	355142	7	NULL	NULL	0	NULL	quetiapine	Chemical	beneficial effect of	is due to					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Although the mechanism of action of quetiapine is unknown, like other anti-psychotics, it inhibits communication between nerves of the brain. It does this by blocking receptors on the nerves for several neurotransmitters, the chemicals that nerves use to communicate with each other. It is thought that its beneficial effect is due to blocking of the dopamine type 2 (D2) and serotonin type 2 (5-HT2) receptors. 	topic_bd
75606	1	355145	7	NULL	NULL	0	NULL	HIF-1α	GP	expression of	is associated with					VEGF	GP	expression of			NULL		0	NULL	NULL	NULL	NULL	NULL	HIF-1α expression is associated with VEGF expression and angiogenesis in colorectal carcinoma.	topic_ccc
75607	2	355145	7	NULL	NULL	0	NULL	HIF-1α	GP	expression of	is associated with					angiogenesis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	HIF-1α expression is associated with VEGF expression and angiogenesis in colorectal carcinoma.	topic_ccc
75608	3	355145	7	NULL	NULL	0	NULL	statement 1	Process		occur in					colorectal carcinoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	HIF-1α expression is associated with VEGF expression and angiogenesis in colorectal carcinoma.	topic_ccc
75609	4	355145	7	NULL	NULL	0	NULL	statement 2	Process		occur in					colorectal carcinoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	HIF-1α expression is associated with VEGF expression and angiogenesis in colorectal carcinoma.	topic_ccc
75633	1	355146	7	NULL	NULL	0	NULL	Neuroleptic	Chemical		refers to					antipsychotic drugs	Chemical	effects of			NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroleptic: A term that refers to the effects of antipsychotic drugs on a patient, especially on his or her cognition and behavior.	topic_bd
75634	2	355146	7	NULL	NULL	0	NULL	statement 1	Process		effect					patients cognition	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroleptic: A term that refers to the effects of antipsychotic drugs on a patient, especially on his or her cognition and behavior.	topic_bd
75635	3	355146	7	NULL	NULL	0	NULL	statement 1	Process		effect					patient behavior	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroleptic: A term that refers to the effects of antipsychotic drugs on a patient, especially on his or her cognition and behavior.	topic_bd
75636	1	355147	7	NULL	NULL	0	NULL	TD	MedicalFinding	persistent	is seen among					neuroleptic-treated bipolar patients	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	There appears to be a significant risk of persistent TD among neuroleptic-treated bipolar patients	topic_bd
75637	1	355149	7	NULL	NULL	0	NULL	HIF-1α 	GP	expression of	is associated with					angiogenesis	Process				NULL	tumor tissue	0	NULL	NULL	NULL	NULL	NULL	 the expression of HIF-1α in tumor tissue is associated with angiogenesis and poor overall survival in patients with colorectal cancer	topic_ccc
75638	2	355149	7	NULL	NULL	0	NULL	HIF-1α 	GP	expression of	is associated with					poor survival	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 the expression of HIF-1α in tumor tissue is associated with angiogenesis and poor overall survival in patients with colorectal cancer	topic_ccc
75639	3	355149	7	NULL	NULL	0	NULL	statement 2	Process		occur in					colorectal cancer patients	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	 the expression of HIF-1α in tumor tissue is associated with angiogenesis and poor overall survival in patients with colorectal cancer	topic_ccc
75640	1	355150	7	NULL	NULL	0	NULL	 smokers	GroupOfPeople		increased risk of					colon cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Ever smokers have an increased risk of colon cancer, which appeared to be more pronounced in the proximal than the distal colon location.	topic_ccc
75641	2	355150	7	NULL	NULL	0	NULL	statement 1	Process		occur in the					proximal colon	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Ever smokers have an increased risk of colon cancer, which appeared to be more pronounced in the proximal than the distal colon location.	topic_ccc
75642	1	355151	7	NULL	NULL	0	NULL	euthymic	MedicalFinding		pertains to					normal mood	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	euthymic, pertaining to a normal mood in which the range of emotions is neither depressed nor highly elevated. NULL	topic_bd
75643	2	355151	7	NULL	NULL	NULL	NULL	euthymic	MedicalFinding		pertains to					depressed	MedicalFinding	emotions which is not			NULL		NULL	NULL	NULL	NULL	NULL	NULL	euthymic, pertaining to a normal mood in which the range of emotions is neither depressed nor highly elevated. NULL	topic_bd
75644	3	355151	7	NULL	NULL	0	NULL	euthymic	MedicalFinding		pertains to					highly elevated	Process	emotions which is not			NULL		0	NULL	NULL	NULL	NULL	NULL	euthymic, pertaining to a normal mood in which the range of emotions is neither depressed nor highly elevated. NULL	topic_bd
75645	4	355151	7	NULL	NULL	0	NULL	statement 2	Process		occur along with					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	euthymic, pertaining to a normal mood in which the range of emotions is neither depressed nor highly elevated. NULL	topic_bd
75646	1	355152	7	NULL	NULL	NULL	NULL	bipolar patients	GroupOfPeople		show					cognitive deficits 	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Previous studies have reported cognitive deficits on tasks of declarative memory in bipolar patients in the euthymic state.	topic_bd
75647	2	355152	7	NULL	NULL	0	NULL	statement 1	Process		occur in					euthymic state	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies have reported cognitive deficits on tasks of declarative memory in bipolar patients in the euthymic state.	topic_bd
75648	1	355153	7	NULL	NULL	0	NULL	Bipolar patients	MedicalFinding		does not perform for					declarative memory	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar patients performed worse than control subjects on a measure of declarative memory (California Verbal Learning Test) but did not differ from the performance of control subjects on either of the two procedural learning tasks (Pursuit Rotor Task and Star Mirror Task).	topic_bd
75649	1	355154	7	NULL	NULL	0	NULL	bipolar disorder persons	GroupOfPeople		has disturbed 					temporal lobe	OrganismPart	function of			NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest disturbed function of temporal lobe, but not basal ganglia, structures in persons with bipolar disorder.	topic_bd
75650	2	355154	7	NULL	NULL	0	NULL	bipolar disorder persons	GroupOfPeople		does not have					basal ganglia	MedicalFinding	disturbance function in			NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest disturbed function of temporal lobe, but not basal ganglia, structures in persons with bipolar disorder.	topic_bd
75651	1	355155	7	NULL	NULL	0	NULL	Physical exercise	PhysicalPhenomenon		maintains					cardiovascular function	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Physical exercise which maintains cardiovascular function can keep the endocrine system in "balance" and is imperative for people with bipolar expression.	topic_bd
75652	2	355155	7	NULL	NULL	0	NULL	statement 1	Process		balance					endocrine system	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Physical exercise which maintains cardiovascular function can keep the endocrine system in "balance" and is imperative for people with bipolar expression.	topic_bd
75653	3	355155	7	NULL	NULL	0	NULL	statement 1	Process		imperative for					bipolar expression 	MedicalFinding	people with			NULL		0	NULL	NULL	NULL	NULL	NULL	Physical exercise which maintains cardiovascular function can keep the endocrine system in "balance" and is imperative for people with bipolar expression.	topic_bd
75654	1	355156	7	NULL	NULL	NULL	NULL	PAPST1 transcripts	GP	 amounts of	is higher than					PAPST2 transcripts	GP	amounts of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	 The relative amount of PAPST1 transcripts was found to be higher than those of PAPST2 in colorectal cancerous tissues.	topic_ccc
75655	2	355156	7	NULL	NULL	0	NULL	statement 1	Process		occur in					colorectal cancerous tissues	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	 The relative amount of PAPST1 transcripts was found to be higher than those of PAPST2 in colorectal cancerous tissues.	topic_ccc
75656	1	355157	7	NULL	NULL	NULL	NULL	PAPS transporter genes	GP		reduce					cellular proteins	GP	extent of sulfation of			NULL	human colorectal carcinoma cells	NULL	NULL	NULL	NULL	NULL	NULL	RNA interference of either of the 2 PAPS transporter genes reduced the extent of sulfation of cellular proteins and cellular proliferation of DLD-1 human colorectal carcinoma cells.	topic_ccc
75657	2	355157	7	NULL	NULL	NULL	NULL	PAPS transporter genes	GP		reduce					DLD-1	Cell	extent of cellular proliferation of			NULL	human colorectal carcinoma cells	NULL	NULL	NULL	NULL	NULL	NULL	RNA interference of either of the 2 PAPS transporter genes reduced the extent of sulfation of cellular proteins and cellular proliferation of DLD-1 human colorectal carcinoma cells.	topic_ccc
74273	1	355158	5	NULL	NULL	0	NULL	pregnancy infection	MedicalFinding	early	confers risk of					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Recent epidemiological studies find that early rather than late pregnancy infection confers the greater risk of schizophrenia.	topic_sch
74274	2	355158	5	NULL	NULL	0	NULL	pregnancy infection	MedicalFinding	late	confers risk of					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Recent epidemiological studies find that early rather than late pregnancy infection confers the greater risk of schizophrenia.	topic_sch
74275	3	355158	5	NULL	NULL	0	NULL	statement 1	Process		is more likely than					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Recent epidemiological studies find that early rather than late pregnancy infection confers the greater risk of schizophrenia.	topic_sch
74321	1	355159	5	NULL	NULL	NULL	NULL	type-1 immune response	AbstractConcept	blunted	is associated with		may			IDO	GP	dysbalance of;;activation of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	In schizophrenia a blunted type-1 immune response seems to be associated with a dysbalance in the activation of the enzyme indoleamine 2,3-dioxygenase (IDO) and in the tryptophan - kynurenine metabolism resulting in increased production of kynurenic acid in schizophrenia.	topic_sch
74322	2	355159	5	NULL	NULL	0	NULL	IDO	GP		is					indoleamine 2,3-dioxygenase	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	In schizophrenia a blunted type-1 immune response seems to be associated with a dysbalance in the activation of the enzyme indoleamine 2,3-dioxygenase (IDO) and in the tryptophan - kynurenine metabolism resulting in increased production of kynurenic acid in schizophrenia.	topic_sch
74323	3	355159	5	NULL	NULL	0	NULL	IDO	GP		is a type of					enzyme	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	In schizophrenia a blunted type-1 immune response seems to be associated with a dysbalance in the activation of the enzyme indoleamine 2,3-dioxygenase (IDO) and in the tryptophan - kynurenine metabolism resulting in increased production of kynurenic acid in schizophrenia.	topic_sch
74324	4	355159	5	NULL	NULL	0	NULL	statement 1	Process		occurs in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In schizophrenia a blunted type-1 immune response seems to be associated with a dysbalance in the activation of the enzyme indoleamine 2,3-dioxygenase (IDO) and in the tryptophan - kynurenine metabolism resulting in increased production of kynurenic acid in schizophrenia.	topic_sch
74325	5	355159	5	NULL	NULL	0	NULL	type-1 immune response	AbstractConcept	blunted	is associated with		may			tryptophan - kynurenine metabolism	Process	dysfunction of			NULL		0	NULL	NULL	NULL	NULL	NULL	In schizophrenia a blunted type-1 immune response seems to be associated with a dysbalance in the activation of the enzyme indoleamine 2,3-dioxygenase (IDO) and in the tryptophan - kynurenine metabolism resulting in increased production of kynurenic acid in schizophrenia.	topic_sch
74326	6	355159	5	NULL	NULL	0	NULL	statement 5	Process		occurs in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In schizophrenia a blunted type-1 immune response seems to be associated with a dysbalance in the activation of the enzyme indoleamine 2,3-dioxygenase (IDO) and in the tryptophan - kynurenine metabolism resulting in increased production of kynurenic acid in schizophrenia.	topic_sch
74327	7	355159	5	NULL	NULL	0	NULL	kynurenic acid	Chemical		is produced in		increased			schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In schizophrenia a blunted type-1 immune response seems to be associated with a dysbalance in the activation of the enzyme indoleamine 2,3-dioxygenase (IDO) and in the tryptophan - kynurenine metabolism resulting in increased production of kynurenic acid in schizophrenia.	topic_sch
74328	8	355159	5	NULL	NULL	0	NULL	statement 1	Process		results in					statement 7	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	In schizophrenia a blunted type-1 immune response seems to be associated with a dysbalance in the activation of the enzyme indoleamine 2,3-dioxygenase (IDO) and in the tryptophan - kynurenine metabolism resulting in increased production of kynurenic acid in schizophrenia.	topic_sch
74329	9	355159	5	NULL	NULL	0	NULL	statement 5	Process		results in					statement 7	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	In schizophrenia a blunted type-1 immune response seems to be associated with a dysbalance in the activation of the enzyme indoleamine 2,3-dioxygenase (IDO) and in the tryptophan - kynurenine metabolism resulting in increased production of kynurenic acid in schizophrenia.	topic_sch
74330	1	355163	5	NULL	NULL	0	NULL	COX-2 inhibitors	Chemical		effects		favourable			schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	COX-2 inhibitors have been tested in clinical trials, pointing to favourable effects in schizophrenia.	topic_sch
74331	1	355165	5	NULL	NULL	NULL	NULL	CB1 receptor	GP	alternation of;;function of	is implicated in					depression	MedicalFinding				NULL	human	NULL	NULL	NULL	NULL	NULL	NULL	Alteration of CB1 receptor function has been implicated in a number of human diseases such as depression, schizophrenia, and obesity (4-6). 	topic_sch
74332	2	355165	5	NULL	NULL	0	NULL	CB1 receptor	GP	alternation of;;function of	is implicated in					schizophrenia	MedicalFinding				NULL	human	0	NULL	NULL	NULL	NULL	NULL	Alteration of CB1 receptor function has been implicated in a number of human diseases such as depression, schizophrenia, and obesity (4-6). 	topic_sch
74333	3	355165	5	NULL	NULL	0	NULL	CB1 receptor	GP	alternation of;;function of	is implicated in					obesity	MedicalFinding				NULL	human	0	NULL	NULL	NULL	NULL	NULL	Alteration of CB1 receptor function has been implicated in a number of human diseases such as depression, schizophrenia, and obesity (4-6). 	topic_sch
74337	1	355166	5	NULL	NULL	0	NULL	PCP	Chemical		is					Phencyclidine	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Phencyclidine (PCP), a noncompetitive N-methyl-D-aspartate (NMDA) receptor antagonist, increases locomotor activity in rodents and causes schizophrenia-like symptoms in humans. 	topic_sch
74338	2	355166	5	NULL	NULL	0	NULL	NMDA	Chemical		is					N-methyl-D-aspartate	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Phencyclidine (PCP), a noncompetitive N-methyl-D-aspartate (NMDA) receptor antagonist, increases locomotor activity in rodents and causes schizophrenia-like symptoms in humans. 	topic_sch
74339	3	355166	5	NULL	NULL	0	NULL	PCP	Chemical		is an antagonist of					NMDA receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Phencyclidine (PCP), a noncompetitive N-methyl-D-aspartate (NMDA) receptor antagonist, increases locomotor activity in rodents and causes schizophrenia-like symptoms in humans. 	topic_sch
74340	4	355166	5	NULL	NULL	0	NULL	PCP	Chemical		increases					locomotor activity	Process				NULL	rodents	0	NULL	NULL	NULL	NULL	NULL	Phencyclidine (PCP), a noncompetitive N-methyl-D-aspartate (NMDA) receptor antagonist, increases locomotor activity in rodents and causes schizophrenia-like symptoms in humans. 	topic_sch
74341	5	355166	5	NULL	NULL	0	NULL	PCP	Chemical		causes					schizophrenia-like symptoms	MedicalFinding				NULL	human	0	NULL	NULL	NULL	NULL	NULL	Phencyclidine (PCP), a noncompetitive N-methyl-D-aspartate (NMDA) receptor antagonist, increases locomotor activity in rodents and causes schizophrenia-like symptoms in humans. 	topic_sch
74342	1	355167	5	NULL	NULL	0	NULL	weight	QuantityOrMeasure	gain of	induced by					antipsychotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The study findings suggest a potential role for leptin to mediate the link between antipsychotic-induced weight gain and beneficial therapeutic response in schizophrenia.	topic_sch
74343	2	355167	5	NULL	NULL	0	NULL	statement 1	QuantityOrMeasure		is linked to					schizophrenia	MedicalFinding	beneficial therapeutic response of			NULL		0	NULL	NULL	NULL	NULL	NULL	The study findings suggest a potential role for leptin to mediate the link between antipsychotic-induced weight gain and beneficial therapeutic response in schizophrenia.	topic_sch
74344	3	355167	5	NULL	NULL	0	NULL	leptin	GP		mediates		may			statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The study findings suggest a potential role for leptin to mediate the link between antipsychotic-induced weight gain and beneficial therapeutic response in schizophrenia.	topic_sch
74345	1	355168	5	NULL	NULL	0	NULL	ADNP	GP		is essential for					brain	OrganismPart	formation of			NULL		0	NULL	NULL	NULL	NULL	NULL	ADNP is essential for brain formation, proper development and neuronal plasticity, all reported to be impaired in schizophrenia. 	topic_sch
74346	2	355168	5	NULL	NULL	0	NULL	ADNP	GP		is essential for					development	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	ADNP is essential for brain formation, proper development and neuronal plasticity, all reported to be impaired in schizophrenia. 	topic_sch
74347	3	355168	5	NULL	NULL	0	NULL	ADNP	GP		is essential for					neuronal plasticity	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	ADNP is essential for brain formation, proper development and neuronal plasticity, all reported to be impaired in schizophrenia. 	topic_sch
74348	4	355168	5	NULL	NULL	0	NULL	brain	OrganismPart	development of	is impaired in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	ADNP is essential for brain formation, proper development and neuronal plasticity, all reported to be impaired in schizophrenia. 	topic_sch
74349	5	355168	5	NULL	NULL	0	NULL	development	Process		is impaired in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	ADNP is essential for brain formation, proper development and neuronal plasticity, all reported to be impaired in schizophrenia. 	topic_sch
74350	6	355168	5	NULL	NULL	0	NULL	neuronal plasticity	Process		is impaired in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	ADNP is essential for brain formation, proper development and neuronal plasticity, all reported to be impaired in schizophrenia. 	topic_sch
74351	1	355169	5	NULL	NULL	0	NULL	ADNP haploinsufficiency	MedicalFinding		inhibits					social function	AbstractConcept				NULL		0	NULL	NULL	NULL	NULL	NULL	ADNP haploinsufficiency inhibits social and cognitive functions, major hallmarks in schizophrenia.	topic_sch
74352	2	355169	5	NULL	NULL	0	NULL	ADNP haploinsufficiency	MedicalFinding		inhibits					cognitive functions	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	ADNP haploinsufficiency inhibits social and cognitive functions, major hallmarks in schizophrenia.	topic_sch
74353	3	355169	5	NULL	NULL	0	NULL	social functions	AbstractConcept	impaired	is a hallmark of					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	ADNP haploinsufficiency inhibits social and cognitive functions, major hallmarks in schizophrenia.	topic_sch
74354	4	355169	5	NULL	NULL	0	NULL	cognitive functions	MentalProcess	impaired	is a hallmark of					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	ADNP haploinsufficiency inhibits social and cognitive functions, major hallmarks in schizophrenia.	topic_sch
74355	1	355171	5	NULL	NULL	0	NULL	ADNP/ADNP2	GP	expression of	is not balanced in					schizophrenia brain	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Imbalance in ADNP/ADNP2 expression in the schizophrenia brain may impact disease progression. 	topic_sch
74356	2	355171	5	NULL	NULL	0	NULL	statement 1	Process		impact		may			schizophrenia spectrum traits	MedicalFinding	progression of			NULL		0	NULL	NULL	NULL	NULL	NULL	Imbalance in ADNP/ADNP2 expression in the schizophrenia brain may impact disease progression. 	topic_sch
74357	1	355174	5	NULL	NULL	0	NULL	serotonin biochemistry regulating gene	GP		cause		may			autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The most likely genes to be candidates for causing autism are those that regulate serotonin biochemistry	topic_aut
74358	1	355176	5	NULL	NULL	0	NULL	serotonin transporter gene	GP		cause		may			autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The serotonin transporter gene has been implicated as a candidate gene in autism owing to the effectiveness of specific drugs that inhibit serotonin transport to minimize some characteristic autistic behaviors.	topic_aut
74359	1	355177	5	NULL	NULL	0	NULL	autism	MedicalFinding		is associated with					serotonin transporter gene	GP	polymorphisms of			NULL		0	NULL	NULL	NULL	NULL	NULL	Cook et al. (1997) reported an association between autism and two distinct polymorphisms of the serotonin transporter gene (HTT)	topic_aut
74360	2	355177	5	NULL	NULL	0	NULL	HTT	GP		is					serotonin transporter gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Cook et al. (1997) reported an association between autism and two distinct polymorphisms of the serotonin transporter gene (HTT)	topic_aut
74361	1	355179	5	NULL	NULL	0	NULL	serotonin	Chemical		is implicated in					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to serotonin, the catecholaminergic neurotransmitters have been implicated in autism.	topic_aut
74362	2	355179	5	NULL	NULL	0	NULL	catecholaminergic neurotransmitters	Chemical		is implicated in					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to serotonin, the catecholaminergic neurotransmitters have been implicated in autism.	topic_aut
74363	1	355180	5	NULL	NULL	NULL	NULL	autism	MedicalFinding		is associated with					HRAS gene marker	GP				NULL		NULL	NULL	NULL	NULL	NULL	NULL	An association has also been found between autism and a marker in the c-harvey ras (HRAS) gene, located on chromosome 11 (Herault et al., 1995).	topic_aut
74364	2	355180	5	NULL	NULL	NULL	NULL	HRAS gene marker	GP		is located on					chromosome 11	Chromosome				NULL		NULL	NULL	NULL	NULL	NULL	NULL	An association has also been found between autism and a marker in the c-harvey ras (HRAS) gene, located on chromosome 11 (Herault et al., 1995).	topic_aut
74365	3	355180	5	NULL	NULL	0	NULL	HRAS gene	GP		is					c-harvey ras gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	An association has also been found between autism and a marker in the c-harvey ras (HRAS) gene, located on chromosome 11 (Herault et al., 1995).	topic_aut
74366	1	355181	5	NULL	NULL	NULL	NULL	HRAS markers	NucleicAcid	region including	confers					autism	MedicalFinding	 susceptibility of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although this association suggests that the region including the HRAS markers confers susceptibility to autism, it is unclear whether the HRAS gene itself, or a gene nearby, is contributing to the autism syndrome (Herault et al., 1995).	topic_aut
74367	1	355182	5	NULL	NULL	0	NULL	15qll-13	Chromosome	duplications of;;small parts of;;the long arm of	plays a role in					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	A number of duplications of small parts of the long arm of chromosome 15 (15qll-13) have been reported in individuals with autism (Baker, Piven, Schwartz, & Patil, 1994), suggesting that a gene may lie in that area.	topic_aut
74368	2	355182	5	NULL	NULL	0	NULL	15qll-13	Chromosome		is present in					chromosome 15	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	A number of duplications of small parts of the long arm of chromosome 15 (15qll-13) have been reported in individuals with autism (Baker, Piven, Schwartz, & Patil, 1994), suggesting that a gene may lie in that area.	topic_aut
76374	1	355183	11	NULL	NULL	0	NULL	Diabetes mellitus	MedicalFinding		is also known as					diabetes	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Diabetes mellitus, often simply referred to as diabetes	topic_mrs
76544	1	355187	11	NULL	NULL	0	NULL	wound	MedicalFinding	open	is at risk of					MRSA infection	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA is especially troublesome in hospitals where patients with open wounds, invasive devices and weakened immune systems are at greater risk of infection than the general public.	topic_mrs
76545	2	355187	11	NULL	NULL	0	NULL	patient with  invasive devices	GroupOfPeople		is at risk of					MRSA infection	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA is especially troublesome in hospitals where patients with open wounds, invasive devices and weakened immune systems are at greater risk of infection than the general public.	topic_mrs
76546	3	355187	11	NULL	NULL	0	NULL	immune system	OrganismPart		is weak in					patients	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA is especially troublesome in hospitals where patients with open wounds, invasive devices and weakened immune systems are at greater risk of infection than the general public.	topic_mrs
76547	4	355187	11	NULL	NULL	0	NULL	statement 3	Process		is at risk of					MRSA infection	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA is especially troublesome in hospitals where patients with open wounds, invasive devices and weakened immune systems are at greater risk of infection than the general public.	topic_mrs
75461	1	355188	11	NULL	NULL	0	NULL	Vancomycin	Chemical		is a type of 					glycopeptide antibiotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Vancomycin  is a glycopeptide antibiotic used in the prophylaxis and treatment of infections caused by Gram-positive bacteria. It has traditionally been reserved as a drug of 'last resort', used only after treatment with other antibiotics had failed	topic_mrs
75462	2	355188	11	NULL	NULL	0	NULL	Gram-positive bacteria	Organism		cause					 infections	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Vancomycin  is a glycopeptide antibiotic used in the prophylaxis and treatment of infections caused by Gram-positive bacteria. It has traditionally been reserved as a drug of 'last resort', used only after treatment with other antibiotics had failed	topic_mrs
75463	3	355188	11	NULL	NULL	0	NULL	Vancomycin	Chemical		used in					 prophylaxis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Vancomycin  is a glycopeptide antibiotic used in the prophylaxis and treatment of infections caused by Gram-positive bacteria. It has traditionally been reserved as a drug of 'last resort', used only after treatment with other antibiotics had failed	topic_mrs
75464	4	355188	11	NULL	NULL	0	NULL	Vancomycin	Chemical		treats					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Vancomycin  is a glycopeptide antibiotic used in the prophylaxis and treatment of infections caused by Gram-positive bacteria. It has traditionally been reserved as a drug of 'last resort', used only after treatment with other antibiotics had failed	topic_mrs
76376	1	355189	11	NULL	NULL	0	NULL	vancomycin	Chemical		is a type of 					 glycopeptide	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	 Linezolid, quinupristin/dalfopristin (synercid), daptomycin, and tigecycline are used to treat more severe infections that do not respond to glycopeptides such as vancomycin.	topic_mrs
76377	2	355189	11	NULL	NULL	0	NULL	severe infections	Process		do not respond to					glycopeptides	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	 Linezolid, quinupristin/dalfopristin (synercid), daptomycin, and tigecycline are used to treat more severe infections that do not respond to glycopeptides such as vancomycin.	topic_mrs
76378	3	355189	11	NULL	NULL	0	NULL	Linezolid	Chemical		treat					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 Linezolid, quinupristin/dalfopristin (synercid), daptomycin, and tigecycline are used to treat more severe infections that do not respond to glycopeptides such as vancomycin.	topic_mrs
76379	4	355189	11	NULL	NULL	0	NULL	quinupristin/dalfopristin	Chemical		treats					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 Linezolid, quinupristin/dalfopristin (synercid), daptomycin, and tigecycline are used to treat more severe infections that do not respond to glycopeptides such as vancomycin.	topic_mrs
76380	5	355189	11	NULL	NULL	0	NULL	daptomycin	Chemical		treats					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 Linezolid, quinupristin/dalfopristin (synercid), daptomycin, and tigecycline are used to treat more severe infections that do not respond to glycopeptides such as vancomycin.	topic_mrs
76381	6	355189	11	NULL	NULL	0	NULL	tigecycline	Chemical		treats					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 Linezolid, quinupristin/dalfopristin (synercid), daptomycin, and tigecycline are used to treat more severe infections that do not respond to glycopeptides such as vancomycin.	topic_mrs
76382	7	355189	11	NULL	NULL	0	NULL	quinupristin/dalfopristin	Chemical		is also known as					synercid	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	 Linezolid, quinupristin/dalfopristin (synercid), daptomycin, and tigecycline are used to treat more severe infections that do not respond to glycopeptides such as vancomycin.	topic_mrs
75465	1	355190	11	NULL	NULL	0	NULL	Gram-positive organisms	Organism		causes					 infections	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Daptomycin is a novel lipopeptide antibiotic used in the treatment of certain infections caused by Gram-positive organisms.	topic_mrs
75466	2	355190	11	NULL	NULL	0	NULL	Daptomycin	Chemical		is a type of 					lipopeptide antibiotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Daptomycin is a novel lipopeptide antibiotic used in the treatment of certain infections caused by Gram-positive organisms.	topic_mrs
75467	3	355190	11	NULL	NULL	0	NULL	Daptomycin	Chemical		treats					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Daptomycin is a novel lipopeptide antibiotic used in the treatment of certain infections caused by Gram-positive organisms.	topic_mrs
76383	1	355191	11	NULL	NULL	0	NULL	methicillin-resistant Staphylococcus aureus 	Organism		is					MRSA	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Rifampicin also has a role in the treatment of methicillin-resistant Staphylococcus aureus (MRSA) in combination with fusidic acid, although recent inquiries have raised questions over the lack of studies into the efficacy of this treatment.	topic_mrs
76384	2	355191	11	NULL	NULL	0	NULL	Rifampicin	Chemical		treats					methicillin-resistant Staphylococcus aureus	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Rifampicin also has a role in the treatment of methicillin-resistant Staphylococcus aureus (MRSA) in combination with fusidic acid, although recent inquiries have raised questions over the lack of studies into the efficacy of this treatment.	topic_mrs
76385	3	355191	11	NULL	NULL	0	NULL	fusidic acid	Chemical		treats					methicillin-resistant Staphylococcus aureus	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Rifampicin also has a role in the treatment of methicillin-resistant Staphylococcus aureus (MRSA) in combination with fusidic acid, although recent inquiries have raised questions over the lack of studies into the efficacy of this treatment.	topic_mrs
76386	4	355191	11	NULL	NULL	0	NULL	statement 2	Chemical		combines with					statement 3	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Rifampicin also has a role in the treatment of methicillin-resistant Staphylococcus aureus (MRSA) in combination with fusidic acid, although recent inquiries have raised questions over the lack of studies into the efficacy of this treatment.	topic_mrs
76387	1	355192	11	NULL	NULL	0	NULL	Community-Acquired MRSA	Organism		is					CA-MRSA	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Community-Acquired MRSA ( CA-MRSA) is a rapidly emerging public health problem. CA-MRSA strains are generally susceptible to a wider range of antibiotics (e.g., usually susceptible to fluoroquinolones and trimethoprim/sulfamethoxazole [TMP/SMX])	topic_mrs
76388	2	355192	11	NULL	NULL	0	NULL	CA-MRSA	Organism		susceptible to		generally			 antibiotics	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Community-Acquired MRSA ( CA-MRSA) is a rapidly emerging public health problem. CA-MRSA strains are generally susceptible to a wider range of antibiotics (e.g., usually susceptible to fluoroquinolones and trimethoprim/sulfamethoxazole [TMP/SMX])	topic_mrs
76389	3	355192	11	NULL	NULL	0	NULL	Community-Acquired MRSA	Organism		susceptible to 					fluoroquinolones	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Community-Acquired MRSA ( CA-MRSA) is a rapidly emerging public health problem. CA-MRSA strains are generally susceptible to a wider range of antibiotics (e.g., usually susceptible to fluoroquinolones and trimethoprim/sulfamethoxazole [TMP/SMX])	topic_mrs
76390	4	355192	11	NULL	NULL	0	NULL	Community-Acquired MRSA	Organism		susceptible to 					trimethoprim/sulfamethoxazole	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Community-Acquired MRSA ( CA-MRSA) is a rapidly emerging public health problem. CA-MRSA strains are generally susceptible to a wider range of antibiotics (e.g., usually susceptible to fluoroquinolones and trimethoprim/sulfamethoxazole [TMP/SMX])	topic_mrs
76391	5	355192	11	NULL	NULL	0	NULL	trimethoprim/sulfamethoxazole	Chemical		is					TMP/SMX	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Community-Acquired MRSA ( CA-MRSA) is a rapidly emerging public health problem. CA-MRSA strains are generally susceptible to a wider range of antibiotics (e.g., usually susceptible to fluoroquinolones and trimethoprim/sulfamethoxazole [TMP/SMX])	topic_mrs
75468	1	355193	11	NULL	NULL	0	NULL	Cellulitis	MedicalFinding		is a type of 					diffuse inflammation	Process	connective tissue			NULL		0	NULL	NULL	NULL	NULL	NULL	Cellulitis is a diffuse inflammation of connective tissue with severe inflammation of dermal and subcutaneous layers of the skin. Cellulitis can be caused by normal skin flora or by exogenous bacteria,	topic_mrs
75469	2	355193	11	NULL	NULL	0	NULL	Cellulitis	MedicalFinding		causes					inflammation	Process	 skin			NULL		0	NULL	NULL	NULL	NULL	NULL	Cellulitis is a diffuse inflammation of connective tissue with severe inflammation of dermal and subcutaneous layers of the skin. Cellulitis can be caused by normal skin flora or by exogenous bacteria,	topic_mrs
75472	3	355193	11	NULL	NULL	0	NULL	Cellulitis	MedicalFinding		caused by		may			normal skin flora	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Cellulitis is a diffuse inflammation of connective tissue with severe inflammation of dermal and subcutaneous layers of the skin. Cellulitis can be caused by normal skin flora or by exogenous bacteria,	topic_mrs
75483	4	355193	11	NULL	NULL	0	NULL	Cellulitis	MedicalFinding		caused by		may			exogenous bacteria	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Cellulitis is a diffuse inflammation of connective tissue with severe inflammation of dermal and subcutaneous layers of the skin. Cellulitis can be caused by normal skin flora or by exogenous bacteria,	topic_mrs
75487	1	355194	11	NULL	NULL	0	NULL	furuncles	MedicalFinding		caused by					S. aureus	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Cellulitis may be caused by numerous organisms that are indigenous to the skin or to particular environmental niches. Cellulitis associated with furuncles, carbuncles, or abscesses is usually caused by S. aureus	topic_mrs
75489	2	355194	11	NULL	NULL	0	NULL	carbuncles	MedicalFinding		caused by					S. aureus	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Cellulitis may be caused by numerous organisms that are indigenous to the skin or to particular environmental niches. Cellulitis associated with furuncles, carbuncles, or abscesses is usually caused by S. aureus	topic_mrs
75490	3	355194	11	NULL	NULL	0	NULL	abscesses	MedicalFinding		caused by					S. aureus	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Cellulitis may be caused by numerous organisms that are indigenous to the skin or to particular environmental niches. Cellulitis associated with furuncles, carbuncles, or abscesses is usually caused by S. aureus	topic_mrs
75491	4	355194	11	NULL	NULL	0	NULL	Cellulitis	MedicalFinding		associated with					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Cellulitis may be caused by numerous organisms that are indigenous to the skin or to particular environmental niches. Cellulitis associated with furuncles, carbuncles, or abscesses is usually caused by S. aureus	topic_mrs
75492	5	355194	11	NULL	NULL	0	NULL	Cellulitis	MedicalFinding		associated with					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Cellulitis may be caused by numerous organisms that are indigenous to the skin or to particular environmental niches. Cellulitis associated with furuncles, carbuncles, or abscesses is usually caused by S. aureus	topic_mrs
75494	6	355194	11	NULL	NULL	0	NULL	Cellulitis	MedicalFinding		associates with					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Cellulitis may be caused by numerous organisms that are indigenous to the skin or to particular environmental niches. Cellulitis associated with furuncles, carbuncles, or abscesses is usually caused by S. aureus	topic_mrs
75498	1	355195	11	NULL	NULL	0	NULL	Impetigo	MedicalFinding		is a type of 					skin infection	Process	 bacterial			NULL		0	NULL	NULL	NULL	NULL	NULL	Impetigo is a highly contagious bacterial skin infection most common among pre-school children	topic_mrs
76623	2	355195	11	NULL	NULL	0	NULL	Impetigo	MedicalFinding		is common among					pre-school children	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Impetigo is a highly contagious bacterial skin infection most common among pre-school children	topic_mrs
76392	1	355200	11	NULL	NULL	0	NULL	Impetigo	MedicalFinding		occurs in		frequently			children	GroupOfPeople	economically disadvantaged			NULL		0	NULL	NULL	NULL	NULL	NULL	Impetigo occurs most frequently among economically disadvantaged children	topic_mrs
76393	1	355201	11	NULL	NULL	0	NULL	streptococcus	Organism		is responsible for					impetigo	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Prospective studies of streptococcal impetigo have demonstrated that the responsible microorganisms initially colonize the unbroken skin, an observation that probably explains the influence of personal hygiene on disease incidence	topic_mrs
76394	2	355201	11	NULL	NULL	0	NULL	streptococcus	Organism		colonizes		initially			unbroken skin	Organism part				NULL		0	NULL	NULL	NULL	NULL	NULL	Prospective studies of streptococcal impetigo have demonstrated that the responsible microorganisms initially colonize the unbroken skin, an observation that probably explains the influence of personal hygiene on disease incidence	topic_mrs
75510	1	355204	11	NULL	NULL	NULL	NULL	Ecthyma	MedicalFinding		is a form of		serious			impetigo	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ecthyma is a more serious form of impetigo in which the infection penetrates deeper into the skin's second layer, the dermis. 	topic_mrs
75511	2	355204	11	NULL	NULL	0	NULL	Ecthyma	MedicalFinding		 infects					 dermis	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Ecthyma is a more serious form of impetigo in which the infection penetrates deeper into the skin's second layer, the dermis. 	topic_mrs
76395	1	355205	11	NULL	NULL	0	NULL	Crystal violet	Chemical		is also known as					Gentian violet	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Crystal violet or Gentian violet (also hexamethyl pararosaniline chloride) is a triarylmethane dye... and was formerly important as a topical antiseptic.	topic_mrs
76396	2	355205	11	NULL	NULL	0	NULL	Crystal violet	Chemical		is a type of 					triarylmethane dye	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Crystal violet or Gentian violet (also hexamethyl pararosaniline chloride) is a triarylmethane dye... and was formerly important as a topical antiseptic.	topic_mrs
76397	3	355205	11	NULL	NULL	0	NULL	hexamethyl pararosaniline chloride	Chemical		is a type of 					triarylmethane dye	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Crystal violet or Gentian violet (also hexamethyl pararosaniline chloride) is a triarylmethane dye... and was formerly important as a topical antiseptic.	topic_mrs
76398	4	355205	11	NULL	NULL	0	NULL	Crystal violet	Chemical		used as		formerly			topical antiseptic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Crystal violet or Gentian violet (also hexamethyl pararosaniline chloride) is a triarylmethane dye... and was formerly important as a topical antiseptic.	topic_mrs
76399	5	355205	11	NULL	NULL	0	NULL	hexamethyl pararosaniline chloride	Chemical		used as		formerly			topical antiseptic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Crystal violet or Gentian violet (also hexamethyl pararosaniline chloride) is a triarylmethane dye... and was formerly important as a topical antiseptic.	topic_mrs
75512	1	355207	11	NULL	NULL	0	NULL	Fusidic acid	Chemical		is a type of 					antibiotic	Chemical	bacteriostatic			NULL		0	NULL	NULL	NULL	NULL	NULL	Fusidic acid is a bacteriostatic antibiotic that is often used topically in creams and eyedrops, but may also be given systemically as tablets or injections	topic_mrs
75513	2	355207	11	NULL	NULL	0	NULL	Fusidic acid	Chemical		is used in					creams	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Fusidic acid is a bacteriostatic antibiotic that is often used topically in creams and eyedrops, but may also be given systemically as tablets or injections	topic_mrs
75514	3	355207	11	NULL	NULL	0	NULL	Fusidic acid	Chemical		is used in					eyedrops	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Fusidic acid is a bacteriostatic antibiotic that is often used topically in creams and eyedrops, but may also be given systemically as tablets or injections	topic_mrs
75515	4	355207	11	NULL	NULL	0	NULL	Fusidic acid	Chemical		is used in		may			 tablets	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Fusidic acid is a bacteriostatic antibiotic that is often used topically in creams and eyedrops, but may also be given systemically as tablets or injections	topic_mrs
75516	5	355207	11	NULL	NULL	0	NULL	Fusidic acid	Chemical		is used in					injection	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Fusidic acid is a bacteriostatic antibiotic that is often used topically in creams and eyedrops, but may also be given systemically as tablets or injections	topic_mrs
76400	1	355208	11	NULL	NULL	0	NULL	fusidic acid	Chemical		is a type of 					bactericidal ointment	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Mild cases may be treated with bactericidal ointment, such as fusidic acid, mupirocin, chloramphenicol or neosporin, which in some countries may be available over-the-counter.	topic_mrs
76401	2	355208	11	NULL	NULL	0	NULL	mupirocin	Chemical		is a type of 					bactericidal ointment	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Mild cases may be treated with bactericidal ointment, such as fusidic acid, mupirocin, chloramphenicol or neosporin, which in some countries may be available over-the-counter.	topic_mrs
76402	3	355208	11	NULL	NULL	0	NULL	chloramphenicol	Chemical		is a type of 					bactericidal ointment	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Mild cases may be treated with bactericidal ointment, such as fusidic acid, mupirocin, chloramphenicol or neosporin, which in some countries may be available over-the-counter.	topic_mrs
76403	4	355208	11	NULL	NULL	0	NULL	neosporin	Chemical		is a type of 					bactericidal ointment	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Mild cases may be treated with bactericidal ointment, such as fusidic acid, mupirocin, chloramphenicol or neosporin, which in some countries may be available over-the-counter.	topic_mrs
76404	1	355209	11	NULL	NULL	0	NULL	Neosporin	Chemical		prevents					 infection	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Neosporin is the product name of an antibiotic ointment produced by Pfizer used in the prevention of infection and speeding the healing of wounds. The original ointment contains three different antibiotics: bacitracin, neomycin, and polymyxin B, in a petroleum jelly base. Other brand names for this mixture include Mycitracin and Topisporin.	topic_mrs
76405	2	355209	11	NULL	NULL	0	NULL	Neosporin	Chemical		heals					wounds	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Neosporin is the product name of an antibiotic ointment produced by Pfizer used in the prevention of infection and speeding the healing of wounds. The original ointment contains three different antibiotics: bacitracin, neomycin, and polymyxin B, in a petroleum jelly base. Other brand names for this mixture include Mycitracin and Topisporin.	topic_mrs
76406	3	355209	11	NULL	NULL	0	NULL	Neosporin	Chemical		contains					bacitracin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Neosporin is the product name of an antibiotic ointment produced by Pfizer used in the prevention of infection and speeding the healing of wounds. The original ointment contains three different antibiotics: bacitracin, neomycin, and polymyxin B, in a petroleum jelly base. Other brand names for this mixture include Mycitracin and Topisporin.	topic_mrs
76407	4	355209	11	NULL	NULL	0	NULL	Neosporin	Chemical		contains					neomycin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Neosporin is the product name of an antibiotic ointment produced by Pfizer used in the prevention of infection and speeding the healing of wounds. The original ointment contains three different antibiotics: bacitracin, neomycin, and polymyxin B, in a petroleum jelly base. Other brand names for this mixture include Mycitracin and Topisporin.	topic_mrs
76408	5	355209	11	NULL	NULL	0	NULL	Neosporin	Chemical		contains					polymyxin B	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Neosporin is the product name of an antibiotic ointment produced by Pfizer used in the prevention of infection and speeding the healing of wounds. The original ointment contains three different antibiotics: bacitracin, neomycin, and polymyxin B, in a petroleum jelly base. Other brand names for this mixture include Mycitracin and Topisporin.	topic_mrs
76409	6	355209	11	NULL	NULL	0	NULL	Neosporin	Chemical		contains					petroleum jelly base	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Neosporin is the product name of an antibiotic ointment produced by Pfizer used in the prevention of infection and speeding the healing of wounds. The original ointment contains three different antibiotics: bacitracin, neomycin, and polymyxin B, in a petroleum jelly base. Other brand names for this mixture include Mycitracin and Topisporin.	topic_mrs
76410	7	355209	11	NULL	NULL	0	NULL	bacitracin	Chemical		is a type of 					antibiotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Neosporin is the product name of an antibiotic ointment produced by Pfizer used in the prevention of infection and speeding the healing of wounds. The original ointment contains three different antibiotics: bacitracin, neomycin, and polymyxin B, in a petroleum jelly base. Other brand names for this mixture include Mycitracin and Topisporin.	topic_mrs
76411	8	355209	11	NULL	NULL	0	NULL	 neomycin	Chemical		is a type of 					antibiotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Neosporin is the product name of an antibiotic ointment produced by Pfizer used in the prevention of infection and speeding the healing of wounds. The original ointment contains three different antibiotics: bacitracin, neomycin, and polymyxin B, in a petroleum jelly base. Other brand names for this mixture include Mycitracin and Topisporin.	topic_mrs
76412	9	355209	11	NULL	NULL	0	NULL	polymyxin B	Chemical		is a type of 					antibiotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Neosporin is the product name of an antibiotic ointment produced by Pfizer used in the prevention of infection and speeding the healing of wounds. The original ointment contains three different antibiotics: bacitracin, neomycin, and polymyxin B, in a petroleum jelly base. Other brand names for this mixture include Mycitracin and Topisporin.	topic_mrs
76413	10	355209	11	NULL	NULL	0	NULL	statement 3	Chemical		mixtured with					statement 4	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Neosporin is the product name of an antibiotic ointment produced by Pfizer used in the prevention of infection and speeding the healing of wounds. The original ointment contains three different antibiotics: bacitracin, neomycin, and polymyxin B, in a petroleum jelly base. Other brand names for this mixture include Mycitracin and Topisporin.	topic_mrs
76414	11	355209	11	NULL	NULL	0	NULL	statement 10	Chemical		mixtured with					statement 5	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Neosporin is the product name of an antibiotic ointment produced by Pfizer used in the prevention of infection and speeding the healing of wounds. The original ointment contains three different antibiotics: bacitracin, neomycin, and polymyxin B, in a petroleum jelly base. Other brand names for this mixture include Mycitracin and Topisporin.	topic_mrs
76415	12	355209	11	NULL	NULL	0	NULL	statement 11	Chemical		mixtured with					statement 6	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Neosporin is the product name of an antibiotic ointment produced by Pfizer used in the prevention of infection and speeding the healing of wounds. The original ointment contains three different antibiotics: bacitracin, neomycin, and polymyxin B, in a petroleum jelly base. Other brand names for this mixture include Mycitracin and Topisporin.	topic_mrs
76416	13	355209	11	NULL	NULL	0	NULL	statement 12	Chemical		also known as					Mycitracin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Neosporin is the product name of an antibiotic ointment produced by Pfizer used in the prevention of infection and speeding the healing of wounds. The original ointment contains three different antibiotics: bacitracin, neomycin, and polymyxin B, in a petroleum jelly base. Other brand names for this mixture include Mycitracin and Topisporin.	topic_mrs
76417	14	355209	11	NULL	NULL	0	NULL	statement 12	Chemical		is also known as					Topisporin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Neosporin is the product name of an antibiotic ointment produced by Pfizer used in the prevention of infection and speeding the healing of wounds. The original ointment contains three different antibiotics: bacitracin, neomycin, and polymyxin B, in a petroleum jelly base. Other brand names for this mixture include Mycitracin and Topisporin.	topic_mrs
76418	1	355211	11	NULL	NULL	0	NULL	Hydrogen peroxide	Chemical		is viscous than		slightly			water	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogen peroxide is a clear liquid, slightly more viscous than water, that appears colorless in dilute solution. It is used as a disinfectant, antiseptic	topic_mrs
76419	2	355211	11	NULL	NULL	0	NULL	Hydrogen peroxide	Chemical		is used as					disinfectant	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogen peroxide is a clear liquid, slightly more viscous than water, that appears colorless in dilute solution. It is used as a disinfectant, antiseptic	topic_mrs
76420	3	355211	11	NULL	NULL	0	NULL	Hydrogen peroxide	Chemical		is used as					antiseptic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogen peroxide is a clear liquid, slightly more viscous than water, that appears colorless in dilute solution. It is used as a disinfectant, antiseptic	topic_mrs
75517	1	355212	11	NULL	NULL	NULL	NULL	Hydrogen peroxide	Chemical		treats					Impetigo Contagiosa	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hydrogen peroxide is an alternative to topical antibiotics in the treatment of Impetigo. In a cream formulation hydrogen peroxide 1% is stabilized, thereby avoiding fast degradation with the result of prolonged antimicrobial effect and effective treatment. Hydrogen peroxide has been shown to be as effective as antibiotics in the treatment of Impetigo Contagiosa.	topic_mrs
76624	2	355212	11	NULL	NULL	0	NULL	Hydrogen peroxide	Chemical		is an alternative to					topical antibiotics	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogen peroxide is an alternative to topical antibiotics in the treatment of Impetigo. In a cream formulation hydrogen peroxide 1% is stabilized, thereby avoiding fast degradation with the result of prolonged antimicrobial effect and effective treatment. Hydrogen peroxide has been shown to be as effective as antibiotics in the treatment of Impetigo Contagiosa.	topic_mrs
74546	1	355213	6	NULL	NULL	0	NULL	HER2 protein	GP		is a type of					HER2 receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The HER2 protein, also called the HER2 receptor	topic_bc
74547	1	355214	6	NULL	NULL	0	NULL	Herceptin	Chemical		is a type of					trastuzumab	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Herceptin (trastuzumab) is part of a treatment plan for the adjuvant treatment of patients with HER2 overexpressing, node-positive HER2+ breast cancer	topic_bc
74548	2	355214	6	NULL	NULL	NULL	NULL	Herceptin	Chemical		is a treatment for					HER2+ breast cancer	MedicalFinding				NULL	patients	NULL	NULL	NULL	NULL	NULL	NULL	Herceptin (trastuzumab) is part of a treatment plan for the adjuvant treatment of patients with HER2 overexpressing, node-positive HER2+ breast cancer	topic_bc
74559	1	355215	6	NULL	NULL	0	NULL	anthracyclines	Chemical		is used as a treatment for					breast cancer	MedicalFinding				NULL	women	0	NULL	NULL	NULL	NULL	NULL	For decades, anthracyclines have been the gold standard of treatment for women with breast cancer, but that could be changing.	topic_bc
74560	1	355216	6	NULL	NULL	NULL	NULL	HER2/ER	GP		cross talk with					lapatinib	Chemical				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Interruption of HER2/ER cross-talk with lapatinib can restore sensitivity to anti-estrogens	topic_bc
74561	2	355216	6	NULL	NULL	0	NULL	statement 1	Process	interruption of	restore					anti-estrogens	Chemical	sensitivity to			NULL		0	NULL	NULL	NULL	NULL	NULL	Interruption of HER2/ER cross-talk with lapatinib can restore sensitivity to anti-estrogens	topic_bc
74562	1	355217	6	NULL	NULL	0	NULL	radiotherapy	MedicalProcedure		prevents					breast cancer	MedicalFinding	recurrence of			NULL	patients	0	NULL	NULL	NULL	NULL	NULL	 After surgery and standard radiotherapy, an extra boost of radiotherapy can help prevent the recurrence of early breast cancer for patients	topic_bc
74563	1	355218	6	NULL	NULL	0	NULL	CtBP1	GP	stablization of 	is dependent on					Bcl3	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Bcl3-dependent stabilization of CtBP1 is crucial for the inhibition of apoptosis and tumor progression in breast cancer.	topic_bc
74564	2	355218	6	NULL	NULL	0	NULL	statement 1	Process		is crucial for					apoptosis	Process				NULL	breast cancer	0	NULL	NULL	NULL	NULL	NULL	Bcl3-dependent stabilization of CtBP1 is crucial for the inhibition of apoptosis and tumor progression in breast cancer.	topic_bc
74565	3	355218	6	NULL	NULL	0	NULL	statement 1	Process		is crucial for					tumor	Cell	progression of 			NULL	breast cancer	0	NULL	NULL	NULL	NULL	NULL	Bcl3-dependent stabilization of CtBP1 is crucial for the inhibition of apoptosis and tumor progression in breast cancer.	topic_bc
74566	1	355219	6	NULL	NULL	0	NULL	quercetin	Chemical		help in					cancer	MedicalFinding	prevention of			NULL		0	NULL	NULL	NULL	NULL	NULL	Research has shown quercetin may help to prevent cancer	topic_bc
74567	1	355220	6	NULL	NULL	NULL	NULL	mucinous carcinoma	MedicalFinding		is a type of		rare			breast cancer	MedicalFinding	invasive			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mucinous (colloid) carcinoma is a rare type of invasive breast cancer that is formed when cancer cells within your breast produce mucous	topic_bc
74568	2	355220	6	NULL	NULL	0	NULL	mucinous carcinoma	MedicalFinding		is a type of					colloid carcinoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mucinous (colloid) carcinoma is a rare type of invasive breast cancer that is formed when cancer cells within your breast produce mucous	topic_bc
74581	3	355220	6	NULL	NULL	0	NULL	breast	CellComponent		produce					mucosa	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Mucinous (colloid) carcinoma is a rare type of invasive breast cancer that is formed when cancer cells within your breast produce mucous	topic_bc
74584	4	355220	6	NULL	NULL	0	NULL	statement 1	Process		is due to					statement 3	process				NULL		0	NULL	NULL	NULL	NULL	NULL	Mucinous (colloid) carcinoma is a rare type of invasive breast cancer that is formed when cancer cells within your breast produce mucous	topic_bc
74589	1	355221	6	NULL	NULL	NULL	NULL	TNC	GP		is involved in					breast cancer	MedicalFinding	metastatic			NULL		NULL	NULL	NULL	NULL	NULL	NULL	TNC is just one gene involved in metastatic breast cancer	topic_bc
74594	1	355222	6	NULL	NULL	0	NULL	IBC			is					Inflammatory breast cancer					NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammatory breast cancer (IBC) is rare	topic_bc
76548	1	355223	11	NULL	NULL	0	NULL	nose	Organism part	skin of	is infected by		actively			MRSA	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Often, MRSA will live somewhat harmlessly in the nasal passages of people who have had previous infections or who work in hospital environments. Less commonly, MRSA will cause active infections in the skin of the nose.	topic_mrs
75560	1	355224	11	NULL	NULL	NULL	NULL	Cutaneous abscesses	MedicalFinding		are collections of					pus	AbstractConcept	dermis;;deeper skin tissues			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cutaneous abscesses are collections of pus within the dermis and deeper skin tissues.S. aureus is present, usually as a single pathogen, in only ∼25% of cutaneous abscesses overall.	topic_mrs
75561	2	355224	11	NULL	NULL	0	NULL	S. aureus	Organism		causes		possibly			statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Cutaneous abscesses are collections of pus within the dermis and deeper skin tissues.S. aureus is present, usually as a single pathogen, in only ∼25% of cutaneous abscesses overall.	topic_mrs
75562	1	355226	11	NULL	NULL	0	NULL	Furuncles	MedicalFinding		infects					hair follicle	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Furuncles (or “boils”) are infections of the hair follicle, usually caused by S. aureus, in which suppuration extends through the dermis into the subcutaneous tissue, where a small abscess forms	topic_mrs
75563	2	355226	11	NULL	NULL	0	NULL	 S. aureus	Organism		causes					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Furuncles (or “boils”) are infections of the hair follicle, usually caused by S. aureus, in which suppuration extends through the dermis into the subcutaneous tissue, where a small abscess forms	topic_mrs
75564	3	355226	11	NULL	NULL	0	NULL	Furuncles	MedicalFinding		associates with					suppuration	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Furuncles (or “boils”) are infections of the hair follicle, usually caused by S. aureus, in which suppuration extends through the dermis into the subcutaneous tissue, where a small abscess forms	topic_mrs
76421	1	355227	11	NULL	NULL	0	NULL	furuncles	MedicalFinding		promotes					drainage	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	For small furuncles, moist heat, which seems to promote drainage, is satisfactory	topic_mrs
76422	1	355228	11	NULL	NULL	0	NULL	Larger furuncles	MedicalFinding		require					 incision	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Larger furuncles and all carbuncles require incision and drainage	topic_mrs
76423	2	355228	11	NULL	NULL	0	NULL	Larger furuncles	MedicalFinding		require					drainage	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Larger furuncles and all carbuncles require incision and drainage	topic_mrs
76424	3	355228	11	NULL	NULL	0	NULL	statement 1	Process		occurs along with					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Larger furuncles and all carbuncles require incision and drainage	topic_mrs
76425	4	355228	11	NULL	NULL	0	NULL	carbuncles	MedicalFinding		require					incision	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Larger furuncles and all carbuncles require incision and drainage	topic_mrs
76426	5	355228	11	NULL	NULL	0	NULL	carbuncles	MedicalFinding		require					drainage	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Larger furuncles and all carbuncles require incision and drainage	topic_mrs
76427	6	355228	11	NULL	NULL	0	NULL	statement 4	Process		occurs along with					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Larger furuncles and all carbuncles require incision and drainage	topic_mrs
75565	1	355229	11	NULL	NULL	NULL	NULL	Carbuncles	MedicalFinding		develop on		tend to			neck	OrganismPart	back of 			NULL		NULL	NULL	NULL	NULL	NULL	NULL	a coalescent inflammatory mass with pus draining from multiple follicular orifices, the lesion is called a carbuncle. Carbuncles tend to develop on the back of the neck and are especially likely to occur in diabetic persons.	topic_mrs
75566	2	355229	11	NULL	NULL	0	NULL	statement 1	Process		occur in		likely 			diabetic persons	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	a coalescent inflammatory mass with pus draining from multiple follicular orifices, the lesion is called a carbuncle. Carbuncles tend to develop on the back of the neck and are especially likely to occur in diabetic persons.	topic_mrs
75567	3	355229	11	NULL	NULL	0	NULL	carbuncle	MedicalFinding		is a type of 					 lesion	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	a coalescent inflammatory mass with pus draining from multiple follicular orifices, the lesion is called a carbuncle. Carbuncles tend to develop on the back of the neck and are especially likely to occur in diabetic persons.	topic_mrs
76428	1	355232	11	NULL	NULL	0	NULL	fomite	Chemical		carries					infectious organisms	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	A fomite is any inanimate object or substance capable of carrying infectious organisms (such as germs or parasites) and hence transferring them from one individual to another. A fomite can be anything (such as a cloth or mop head), so when cleaning, it is important to remember that such items could aid the spread of pathogenic organisms. Skin cells, hair, clothing, and bedding are common hospital sources of contamination.	topic_mrs
76429	2	355232	11	NULL	NULL	0	NULL	germs	Organism		is a type of 					 infectious organisms	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	A fomite is any inanimate object or substance capable of carrying infectious organisms (such as germs or parasites) and hence transferring them from one individual to another. A fomite can be anything (such as a cloth or mop head), so when cleaning, it is important to remember that such items could aid the spread of pathogenic organisms. Skin cells, hair, clothing, and bedding are common hospital sources of contamination.	topic_mrs
76430	3	355232	11	NULL	NULL	0	NULL	parasites	Organism		is a type of 					infectious organisms	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	A fomite is any inanimate object or substance capable of carrying infectious organisms (such as germs or parasites) and hence transferring them from one individual to another. A fomite can be anything (such as a cloth or mop head), so when cleaning, it is important to remember that such items could aid the spread of pathogenic organisms. Skin cells, hair, clothing, and bedding are common hospital sources of contamination.	topic_mrs
76431	4	355232	11	NULL	NULL	0	NULL	cloth	Chemical		is a type of 					fomite	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	A fomite is any inanimate object or substance capable of carrying infectious organisms (such as germs or parasites) and hence transferring them from one individual to another. A fomite can be anything (such as a cloth or mop head), so when cleaning, it is important to remember that such items could aid the spread of pathogenic organisms. Skin cells, hair, clothing, and bedding are common hospital sources of contamination.	topic_mrs
76432	5	355232	11	NULL	NULL	0	NULL	mop head	Chemical		is a type of 					fomite	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	A fomite is any inanimate object or substance capable of carrying infectious organisms (such as germs or parasites) and hence transferring them from one individual to another. A fomite can be anything (such as a cloth or mop head), so when cleaning, it is important to remember that such items could aid the spread of pathogenic organisms. Skin cells, hair, clothing, and bedding are common hospital sources of contamination.	topic_mrs
76433	6	355232	11	NULL	NULL	0	NULL	Skin cells	Cell		are source of 		common			hospital contamination	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	A fomite is any inanimate object or substance capable of carrying infectious organisms (such as germs or parasites) and hence transferring them from one individual to another. A fomite can be anything (such as a cloth or mop head), so when cleaning, it is important to remember that such items could aid the spread of pathogenic organisms. Skin cells, hair, clothing, and bedding are common hospital sources of contamination.	topic_mrs
76434	7	355232	11	NULL	NULL	0	NULL	hair	OrganismPart		are source of		common			hospital contamination					NULL		0	NULL	NULL	NULL	NULL	NULL	A fomite is any inanimate object or substance capable of carrying infectious organisms (such as germs or parasites) and hence transferring them from one individual to another. A fomite can be anything (such as a cloth or mop head), so when cleaning, it is important to remember that such items could aid the spread of pathogenic organisms. Skin cells, hair, clothing, and bedding are common hospital sources of contamination.	topic_mrs
76435	8	355232	11	NULL	NULL	0	NULL	clothing	Chemical		are source of		common			hospital contamination	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	A fomite is any inanimate object or substance capable of carrying infectious organisms (such as germs or parasites) and hence transferring them from one individual to another. A fomite can be anything (such as a cloth or mop head), so when cleaning, it is important to remember that such items could aid the spread of pathogenic organisms. Skin cells, hair, clothing, and bedding are common hospital sources of contamination.	topic_mrs
76436	9	355232	11	NULL	NULL	0	NULL	bedding	Chemical		are source of		common			hospital contamination	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	A fomite is any inanimate object or substance capable of carrying infectious organisms (such as germs or parasites) and hence transferring them from one individual to another. A fomite can be anything (such as a cloth or mop head), so when cleaning, it is important to remember that such items could aid the spread of pathogenic organisms. Skin cells, hair, clothing, and bedding are common hospital sources of contamination.	topic_mrs
76437	1	355233	11	NULL	NULL	0	NULL	chlorhexidine	Chemical		is a type of 					 antibacterial soaps	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	In some cases, fomites may harbor the organism and facilitate transmission of the infection. Depending on the individual circumstances, control of outbreaks may require bathing with antibacterial soaps, such as chlorhexidine; thorough laundering of clothing, towels, and bed wear; separate use of towels and washcloths; and attempted eradication of staphylococcal carriage among colonized persons.	topic_mrs
76438	2	355233	11	NULL	NULL	0	NULL	fomites	Chemical		harbor		may			organism 	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	In some cases, fomites may harbor the organism and facilitate transmission of the infection. Depending on the individual circumstances, control of outbreaks may require bathing with antibacterial soaps, such as chlorhexidine; thorough laundering of clothing, towels, and bed wear; separate use of towels and washcloths; and attempted eradication of staphylococcal carriage among colonized persons.	topic_mrs
76439	3	355233	11	NULL	NULL	0	NULL	fomites	Chemical		transmit					infection	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	In some cases, fomites may harbor the organism and facilitate transmission of the infection. Depending on the individual circumstances, control of outbreaks may require bathing with antibacterial soaps, such as chlorhexidine; thorough laundering of clothing, towels, and bed wear; separate use of towels and washcloths; and attempted eradication of staphylococcal carriage among colonized persons.	topic_mrs
76440	1	355235	11	NULL	NULL	0	NULL	mupirocin ointment	Chemical		treats					nasal colonization	Process	anterior nares			NULL		0	NULL	NULL	NULL	NULL	NULL	For persons with nasal colonization, one approach is the application of mupirocin ointment twice daily in the anterior nares for the first 5 days each month. This regimen reduces recurrences by ∼50%.	topic_mrs
76441	2	355235	11	NULL	NULL	0	NULL	statement 1	Process		reduces					recurrence	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	For persons with nasal colonization, one approach is the application of mupirocin ointment twice daily in the anterior nares for the first 5 days each month. This regimen reduces recurrences by ∼50%.	topic_mrs
75568	1	355236	11	NULL	NULL	0	NULL	S. aureus	Organism		causes					furunculosis	MedicalFinding	recurrent			NULL		0	NULL	NULL	NULL	NULL	NULL	Clindamycin is an exception, and probably the best program for recurrent furunculosis caused by susceptible S. aureus is a single oral daily dose of 150 mg of this agent for 3 months, which decreases subsequent infections by ∼80%.	topic_mrs
75569	2	355236	11	NULL	NULL	0	NULL	Clindamycin	Chemical		treats		probably			statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Clindamycin is an exception, and probably the best program for recurrent furunculosis caused by susceptible S. aureus is a single oral daily dose of 150 mg of this agent for 3 months, which decreases subsequent infections by ∼80%.	topic_mrs
76442	1	355237	11	NULL	NULL	0	NULL	Erysipelas	MedicalFinding		is a type of 					cutaneous infection	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Erysipelas is distinguished clinically from other forms of cutaneous infection by the following 2 features: the lesions are raised above the level of the surrounding skin, and there is a clear line of demarcation between involved and uninvolved tissue...Rarely, group B streptococci or S. aureus may be involved.	topic_mrs
76443	2	355237	11	NULL	NULL	0	NULL	B streptococci	Organism		involved in		may			Erysipelas	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Erysipelas is distinguished clinically from other forms of cutaneous infection by the following 2 features: the lesions are raised above the level of the surrounding skin, and there is a clear line of demarcation between involved and uninvolved tissue...Rarely, group B streptococci or S. aureus may be involved.	topic_mrs
76444	3	355237	11	NULL	NULL	0	NULL	S. aureus	Organism		involved in		may			Erysipelas	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Erysipelas is distinguished clinically from other forms of cutaneous infection by the following 2 features: the lesions are raised above the level of the surrounding skin, and there is a clear line of demarcation between involved and uninvolved tissue...Rarely, group B streptococci or S. aureus may be involved.	topic_mrs
75570	1	355238	11	NULL	NULL	0	NULL	erysipelas	MedicalFinding		is also known as					Holy Fire	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	erysipelas is an acute streptococcus bacterial infection of the dermis, resulting in inflammation. It is also known as Holy Fire 	topic_mrs
75573	2	355238	11	NULL	NULL	NULL	NULL	erysipelas	MedicalFinding		is a type of 					acute streptococcus bacterial infection	MedicalFinding	of dermis			NULL		NULL	NULL	NULL	NULL	NULL	NULL	erysipelas is an acute streptococcus bacterial infection of the dermis, resulting in inflammation. It is also known as Holy Fire 	topic_mrs
75574	3	355238	11	NULL	NULL	0	NULL	statement 2	Process		resulting in					inflammation	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	erysipelas is an acute streptococcus bacterial infection of the dermis, resulting in inflammation. It is also known as Holy Fire 	topic_mrs
76445	1	355241	11	NULL	NULL	0	NULL	saphenous venectomy	MedicalProcedure		is a type of 					Surgical procedure	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Surgical procedures that increase the risk for cellulitis, presumably due to disruption of lymphatic drainage, include saphenous venectomy, axillary node dissection for breast cancer, and operations for gynecologic malignancies that involve lymph node dissection, especially when followed by radiation therapy, such as radical vulvectomy and radical hysterectomy	topic_mrs
76446	2	355241	11	NULL	NULL	0	NULL	axillary node dissection	MedicalFinding	for breast cancer	is a type of 					Surgical procedure	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Surgical procedures that increase the risk for cellulitis, presumably due to disruption of lymphatic drainage, include saphenous venectomy, axillary node dissection for breast cancer, and operations for gynecologic malignancies that involve lymph node dissection, especially when followed by radiation therapy, such as radical vulvectomy and radical hysterectomy	topic_mrs
76447	3	355241	11	NULL	NULL	0	NULL	lymph node dissection	MedicalFinding		is a type of 					Surgical procedure	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Surgical procedures that increase the risk for cellulitis, presumably due to disruption of lymphatic drainage, include saphenous venectomy, axillary node dissection for breast cancer, and operations for gynecologic malignancies that involve lymph node dissection, especially when followed by radiation therapy, such as radical vulvectomy and radical hysterectomy	topic_mrs
76448	4	355241	11	NULL	NULL	0	NULL	radical vulvectomy	MedicalFinding		is a type of 					radiation therapy	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Surgical procedures that increase the risk for cellulitis, presumably due to disruption of lymphatic drainage, include saphenous venectomy, axillary node dissection for breast cancer, and operations for gynecologic malignancies that involve lymph node dissection, especially when followed by radiation therapy, such as radical vulvectomy and radical hysterectomy	topic_mrs
76449	5	355241	11	NULL	NULL	0	NULL	radical hysterectomy	MedicalFinding		is a type of 					radiation therapy	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Surgical procedures that increase the risk for cellulitis, presumably due to disruption of lymphatic drainage, include saphenous venectomy, axillary node dissection for breast cancer, and operations for gynecologic malignancies that involve lymph node dissection, especially when followed by radiation therapy, such as radical vulvectomy and radical hysterectomy	topic_mrs
76450	6	355241	11	NULL	NULL	0	NULL	saphenous venectomy	MedicalFinding		 increase					cellulitis	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Surgical procedures that increase the risk for cellulitis, presumably due to disruption of lymphatic drainage, include saphenous venectomy, axillary node dissection for breast cancer, and operations for gynecologic malignancies that involve lymph node dissection, especially when followed by radiation therapy, such as radical vulvectomy and radical hysterectomy	topic_mrs
76451	7	355241	11	NULL	NULL	0	NULL	axillary node dissection	MedicalFinding		increases					 cellulitis	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Surgical procedures that increase the risk for cellulitis, presumably due to disruption of lymphatic drainage, include saphenous venectomy, axillary node dissection for breast cancer, and operations for gynecologic malignancies that involve lymph node dissection, especially when followed by radiation therapy, such as radical vulvectomy and radical hysterectomy	topic_mrs
76452	8	355241	11	NULL	NULL	0	NULL	lymph node dissection	MedicalFinding		increases					cellulitis	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Surgical procedures that increase the risk for cellulitis, presumably due to disruption of lymphatic drainage, include saphenous venectomy, axillary node dissection for breast cancer, and operations for gynecologic malignancies that involve lymph node dissection, especially when followed by radiation therapy, such as radical vulvectomy and radical hysterectomy	topic_mrs
76453	9	355241	11	NULL	NULL	0	NULL	radical vulvectomy	MedicalFinding		increases					cellulitis	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Surgical procedures that increase the risk for cellulitis, presumably due to disruption of lymphatic drainage, include saphenous venectomy, axillary node dissection for breast cancer, and operations for gynecologic malignancies that involve lymph node dissection, especially when followed by radiation therapy, such as radical vulvectomy and radical hysterectomy	topic_mrs
76454	10	355241	11	NULL	NULL	0	NULL	radical hysterectomy	MedicalFinding		increases					cellulitis	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Surgical procedures that increase the risk for cellulitis, presumably due to disruption of lymphatic drainage, include saphenous venectomy, axillary node dissection for breast cancer, and operations for gynecologic malignancies that involve lymph node dissection, especially when followed by radiation therapy, such as radical vulvectomy and radical hysterectomy	topic_mrs
75610	1	355243	11	NULL	NULL	0	NULL	Necrosis	MedicalFinding		means					 premature death	Process	cells;;living tissue			NULL		0	NULL	NULL	NULL	NULL	NULL	Necrosis is the premature death of cells and living tissue. Necrosis is caused by factors external to the cell or tissue, such as infection, toxins, or trauma. 	topic_mrs
75611	2	355243	11	NULL	NULL	0	NULL	Necrosis	MedicalFinding		caused by					infection	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Necrosis is the premature death of cells and living tissue. Necrosis is caused by factors external to the cell or tissue, such as infection, toxins, or trauma. 	topic_mrs
75612	3	355243	11	NULL	NULL	0	NULL	Necrosis	MedicalFinding		caused by					toxins	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Necrosis is the premature death of cells and living tissue. Necrosis is caused by factors external to the cell or tissue, such as infection, toxins, or trauma. 	topic_mrs
75613	4	355243	11	NULL	NULL	0	NULL	Necrosis	MedicalFinding		caused by					trauma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Necrosis is the premature death of cells and living tissue. Necrosis is caused by factors external to the cell or tissue, such as infection, toxins, or trauma. 	topic_mrs
76455	1	355244	11	NULL	NULL	NULL	NULL	Debridement	MedicalProcedure		is removal of 		 medical 			dead tissues	OrganismPart				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Debridement is the medical removal of a patient's dead, damaged, or infected tissue to improve the healing potential of the remaining healthy tissue	topic_mrs
76456	2	355244	11	NULL	NULL	NULL	NULL	Debridement	MedicalProcedure		is removal of 					dead tissues	Organism part				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Debridement is the medical removal of a patient's dead, damaged, or infected tissue to improve the healing potential of the remaining healthy tissue	topic_mrs
76457	3	355244	11	NULL	NULL	NULL	NULL	Debridement	MedicalProcedure		is removal of					dead tissues	Organism part				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Debridement is the medical removal of a patient's dead, damaged, or infected tissue to improve the healing potential of the remaining healthy tissue	topic_mrs
76458	4	355244	11	NULL	NULL	NULL	NULL	statement 1	Process		improve					healthy tissues	OrganismPart	healing potential of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Debridement is the medical removal of a patient's dead, damaged, or infected tissue to improve the healing potential of the remaining healthy tissue	topic_mrs
76459	5	355244	11	NULL	NULL	NULL	NULL	statement 2	Process		improve					healthy tissue	OrganismPart	healing potential of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Debridement is the medical removal of a patient's dead, damaged, or infected tissue to improve the healing potential of the remaining healthy tissue	topic_mrs
76460	6	355244	11	NULL	NULL	NULL	NULL	statement 3	Process		improve					healthy tissue	OrganismPart	healing potential of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Debridement is the medical removal of a patient's dead, damaged, or infected tissue to improve the healing potential of the remaining healthy tissue	topic_mrs
76461	1	355245	11	NULL	NULL	0	NULL	cefazolin	Chemical		is also known as					cefazoline	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	cefazolin, also known as cefazoline or cephazolin, is a first-generation cephalosporin antibiotic.	topic_mrs
76462	2	355245	11	NULL	NULL	0	NULL	cefazolin	Chemical		is also known as					cephazolin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	cefazolin, also known as cefazoline or cephazolin, is a first-generation cephalosporin antibiotic.	topic_mrs
76463	3	355245	11	NULL	NULL	0	NULL	cefazolin	Chemical		is a type of 					first-generation cephalosporin antibiotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	cefazolin, also known as cefazoline or cephazolin, is a first-generation cephalosporin antibiotic.	topic_mrs
76464	1	355248	11	NULL	NULL	NULL	NULL	Elevation	MedicalProcedure		drains					swollen fluids	Cell Component				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Elevation leads to drainage of swollen fluids, leading to a faster recovery time	topic_mrs
76465	2	355248	11	NULL	NULL	NULL	NULL	statement 1	Process		leading to					recovery	Process	faster			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Elevation leads to drainage of swollen fluids, leading to a faster recovery time	topic_mrs
76466	1	355250	11	NULL	NULL	NULL	NULL	antibiotic solution	Chemical		decrease					wound	MedicalFinding	infection of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	 Irrigation of wounds with antibiotic solutions is associated with decreased rate of wound infection. 	topic_mrs
76467	1	355253	11	NULL	NULL	NULL	NULL	surgical site infection	MedicalFinding		occurs after					surgery	MedicalProcedure				NULL		NULL	NULL	NULL	NULL	NULL	NULL	A surgical site infection is an infection that occurs after surgery in the part of the body where the surgery took place. Most patients who have surgery do not develop an infection. However, infections develop in about 1 to 3 out of every 100 patients who have surgery.	topic_mrs
76549	1	355254	11	NULL	NULL	0	NULL	SSI	medical finding	therapy for	include					incision	medical finding	opening of			NULL		0	NULL	NULL	NULL	NULL	NULL	The primary, and most important, therapy for SSI is to open the incision, evacuate the infected material, and continue dressing changes until the wound heals by secondary intention.	topic_mrs
76550	2	355254	11	NULL	NULL	0	NULL	statement 1	Process		is followed by					infected material	AbstractConcept	evacuation of			NULL		0	NULL	NULL	NULL	NULL	NULL	The primary, and most important, therapy for SSI is to open the incision, evacuate the infected material, and continue dressing changes until the wound heals by secondary intention.	topic_mrs
76551	3	355254	11	NULL	NULL	0	NULL	statement 2	Process		is followed by					dressing	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	The primary, and most important, therapy for SSI is to open the incision, evacuate the infected material, and continue dressing changes until the wound heals by secondary intention.	topic_mrs
76552	4	355254	11	NULL	NULL	0	NULL	wound	MedicalFinding		heals by					secondary intention	medical procedure				NULL		0	NULL	NULL	NULL	NULL	NULL	The primary, and most important, therapy for SSI is to open the incision, evacuate the infected material, and continue dressing changes until the wound heals by secondary intention.	topic_mrs
76553	5	355254	11	NULL	NULL	0	NULL	statement 3	Process		is continued untill					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The primary, and most important, therapy for SSI is to open the incision, evacuate the infected material, and continue dressing changes until the wound heals by secondary intention.	topic_mrs
74369	1	355255	5	NULL	NULL	0	NULL	Rs9722	Chromosome		is a type of					SNP	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	Rs9722 and rs1051169 have been reported as affecting the levels of S100B in the serum or the brain, and haplotypes containing these two SNPs have been associated with schizophrenia.	topic_sch
74370	2	355255	5	NULL	NULL	0	NULL	rs1051169	Chromosome		is a type of					SNP	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	Rs9722 and rs1051169 have been reported as affecting the levels of S100B in the serum or the brain, and haplotypes containing these two SNPs have been associated with schizophrenia.	topic_sch
74371	3	355255	5	NULL	NULL	0	NULL	Rs9722	Chromosome		affects					S100B	GP	level of			NULL	serum	0	NULL	NULL	NULL	NULL	NULL	Rs9722 and rs1051169 have been reported as affecting the levels of S100B in the serum or the brain, and haplotypes containing these two SNPs have been associated with schizophrenia.	topic_sch
74372	4	355255	5	NULL	NULL	0	NULL	Rs9722	Chromosome		affects					S100B	GP	level of			NULL	brain	0	NULL	NULL	NULL	NULL	NULL	Rs9722 and rs1051169 have been reported as affecting the levels of S100B in the serum or the brain, and haplotypes containing these two SNPs have been associated with schizophrenia.	topic_sch
74373	5	355255	5	NULL	NULL	0	NULL	rs1051169	Chromosome		affects					S100B	GP	level of			NULL	serum	0	NULL	NULL	NULL	NULL	NULL	Rs9722 and rs1051169 have been reported as affecting the levels of S100B in the serum or the brain, and haplotypes containing these two SNPs have been associated with schizophrenia.	topic_sch
74374	6	355255	5	NULL	NULL	0	NULL	rs1051169	Chromosome		affects					S100B	GP	level of			NULL	brain	0	NULL	NULL	NULL	NULL	NULL	Rs9722 and rs1051169 have been reported as affecting the levels of S100B in the serum or the brain, and haplotypes containing these two SNPs have been associated with schizophrenia.	topic_sch
74375	7	355255	5	NULL	NULL	0	NULL	haplotype	Chromosome		contains					Rs9722	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	Rs9722 and rs1051169 have been reported as affecting the levels of S100B in the serum or the brain, and haplotypes containing these two SNPs have been associated with schizophrenia.	topic_sch
74376	8	355255	5	NULL	NULL	0	NULL	haplotype	Chromosome		contains					rs1051169	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	Rs9722 and rs1051169 have been reported as affecting the levels of S100B in the serum or the brain, and haplotypes containing these two SNPs have been associated with schizophrenia.	topic_sch
74377	9	355255	5	NULL	NULL	0	NULL	statement 7	Process		occurs along with					statement 8	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Rs9722 and rs1051169 have been reported as affecting the levels of S100B in the serum or the brain, and haplotypes containing these two SNPs have been associated with schizophrenia.	topic_sch
74378	10	355255	5	NULL	NULL	0	NULL	statement 7	Process		is associated with					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Rs9722 and rs1051169 have been reported as affecting the levels of S100B in the serum or the brain, and haplotypes containing these two SNPs have been associated with schizophrenia.	topic_sch
74379	11	355255	5	NULL	NULL	0	NULL	statement 8	Process		is associated with					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Rs9722 and rs1051169 have been reported as affecting the levels of S100B in the serum or the brain, and haplotypes containing these two SNPs have been associated with schizophrenia.	topic_sch
74380	1	355256	5	NULL	NULL	NULL	NULL	S100B gene polymorphism	AbstractConcept		plays a role in					schizophrenia patients	GroupOfPeople	cognitive functions of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results implicate a role for S100B gene polymorphisms in the cognitive functions of schizophrenia patients and encourage further investigation into spatial disability as an endophenotype of schizophrenia.	topic_sch
74381	2	355256	5	NULL	NULL	0	NULL	spatial disability	MedicalFinding		is an endophenotype of					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	These results implicate a role for S100B gene polymorphisms in the cognitive functions of schizophrenia patients and encourage further investigation into spatial disability as an endophenotype of schizophrenia.	topic_sch
75658	1	355257	7	NULL	NULL	0	NULL	mitochondrial respiration	Process	decreased	indicates					mitochondria	CellComponent	dysfunction of			NULL		0	NULL	NULL	NULL	NULL	NULL	Several pieces of evidence point to an underlying dysfunction of mitochondria: (i) decreased mitochondrial respiration; (ii) changes in mitochondrial morphology; (iii) increases in mitochondrial DNA (mtDNA) polymorphisms and in levels of mtDNA mutations; (iv) downregulation of nuclear mRNA molecules and proteins involved in mitochondrial respiration; (v) decreased high-energy phosphates and decreased pH in the brain; and (vi) psychotic and affective symptoms, and cognitive decline in mitochondrial previous termdisorders.next term	topic_bd
75659	2	355257	7	NULL	NULL	0	NULL	mitochondrial morphology	CellComponent	changes in	indicates					mitochondria	CellComponent	dysfunction of			NULL		0	NULL	NULL	NULL	NULL	NULL	Several pieces of evidence point to an underlying dysfunction of mitochondria: (i) decreased mitochondrial respiration; (ii) changes in mitochondrial morphology; (iii) increases in mitochondrial DNA (mtDNA) polymorphisms and in levels of mtDNA mutations; (iv) downregulation of nuclear mRNA molecules and proteins involved in mitochondrial respiration; (v) decreased high-energy phosphates and decreased pH in the brain; and (vi) psychotic and affective symptoms, and cognitive decline in mitochondrial previous termdisorders.next term	topic_bd
75660	3	355257	7	NULL	NULL	0	NULL	mtDNA polymorphisms	NucleicAcid	increase in	indicates					mitochondria	CellComponent	dysfunction of			NULL		0	NULL	NULL	NULL	NULL	NULL	Several pieces of evidence point to an underlying dysfunction of mitochondria: (i) decreased mitochondrial respiration; (ii) changes in mitochondrial morphology; (iii) increases in mitochondrial DNA (mtDNA) polymorphisms and in levels of mtDNA mutations; (iv) downregulation of nuclear mRNA molecules and proteins involved in mitochondrial respiration; (v) decreased high-energy phosphates and decreased pH in the brain; and (vi) psychotic and affective symptoms, and cognitive decline in mitochondrial previous termdisorders.next term	topic_bd
75661	4	355257	7	NULL	NULL	NULL	NULL	mtDNA 	NucleicAcid	increase in;;mutations in	indicates					mitochondria	CellComponent	dysfunction of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Several pieces of evidence point to an underlying dysfunction of mitochondria: (i) decreased mitochondrial respiration; (ii) changes in mitochondrial morphology; (iii) increases in mitochondrial DNA (mtDNA) polymorphisms and in levels of mtDNA mutations; (iv) downregulation of nuclear mRNA molecules and proteins involved in mitochondrial respiration; (v) decreased high-energy phosphates and decreased pH in the brain; and (vi) psychotic and affective symptoms, and cognitive decline in mitochondrial previous termdisorders.next term	topic_bd
75662	5	355257	7	NULL	NULL	NULL	NULL	nuclear mRNA molecules 	NucleicAcid	downregulation of	indicates					mitochondria	CellComponent	dysfunction of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Several pieces of evidence point to an underlying dysfunction of mitochondria: (i) decreased mitochondrial respiration; (ii) changes in mitochondrial morphology; (iii) increases in mitochondrial DNA (mtDNA) polymorphisms and in levels of mtDNA mutations; (iv) downregulation of nuclear mRNA molecules and proteins involved in mitochondrial respiration; (v) decreased high-energy phosphates and decreased pH in the brain; and (vi) psychotic and affective symptoms, and cognitive decline in mitochondrial previous termdisorders.next term	topic_bd
75663	6	355257	7	NULL	NULL	NULL	NULL	nuclear proteins	GP	downregulation of	indicates					mitochondria	CellComponent	dysfunction of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Several pieces of evidence point to an underlying dysfunction of mitochondria: (i) decreased mitochondrial respiration; (ii) changes in mitochondrial morphology; (iii) increases in mitochondrial DNA (mtDNA) polymorphisms and in levels of mtDNA mutations; (iv) downregulation of nuclear mRNA molecules and proteins involved in mitochondrial respiration; (v) decreased high-energy phosphates and decreased pH in the brain; and (vi) psychotic and affective symptoms, and cognitive decline in mitochondrial previous termdisorders.next term	topic_bd
75664	7	355257	7	NULL	NULL	0	NULL	nuclear mRNA molecules 	GP		involved in					mitochondrial respiration	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Several pieces of evidence point to an underlying dysfunction of mitochondria: (i) decreased mitochondrial respiration; (ii) changes in mitochondrial morphology; (iii) increases in mitochondrial DNA (mtDNA) polymorphisms and in levels of mtDNA mutations; (iv) downregulation of nuclear mRNA molecules and proteins involved in mitochondrial respiration; (v) decreased high-energy phosphates and decreased pH in the brain; and (vi) psychotic and affective symptoms, and cognitive decline in mitochondrial previous termdisorders.next term	topic_bd
75665	8	355257	7	NULL	NULL	0	NULL	nuclear proteins	GP		involved in					mitochondrial respiration	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Several pieces of evidence point to an underlying dysfunction of mitochondria: (i) decreased mitochondrial respiration; (ii) changes in mitochondrial morphology; (iii) increases in mitochondrial DNA (mtDNA) polymorphisms and in levels of mtDNA mutations; (iv) downregulation of nuclear mRNA molecules and proteins involved in mitochondrial respiration; (v) decreased high-energy phosphates and decreased pH in the brain; and (vi) psychotic and affective symptoms, and cognitive decline in mitochondrial previous termdisorders.next term	topic_bd
75666	9	355257	7	NULL	NULL	NULL	NULL	high energy phosphates	Chemical	decrease of;;brain	indicates					mitochondria	CellComponent	dysfunction of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Several pieces of evidence point to an underlying dysfunction of mitochondria: (i) decreased mitochondrial respiration; (ii) changes in mitochondrial morphology; (iii) increases in mitochondrial DNA (mtDNA) polymorphisms and in levels of mtDNA mutations; (iv) downregulation of nuclear mRNA molecules and proteins involved in mitochondrial respiration; (v) decreased high-energy phosphates and decreased pH in the brain; and (vi) psychotic and affective symptoms, and cognitive decline in mitochondrial previous termdisorders.next term	topic_bd
75667	10	355257	7	NULL	NULL	0	NULL	pH	PhysicalPhenomenon	decrease of;;brain	indicates					mitochondria	CellComponent	dysfunction of			NULL		0	NULL	NULL	NULL	NULL	NULL	Several pieces of evidence point to an underlying dysfunction of mitochondria: (i) decreased mitochondrial respiration; (ii) changes in mitochondrial morphology; (iii) increases in mitochondrial DNA (mtDNA) polymorphisms and in levels of mtDNA mutations; (iv) downregulation of nuclear mRNA molecules and proteins involved in mitochondrial respiration; (v) decreased high-energy phosphates and decreased pH in the brain; and (vi) psychotic and affective symptoms, and cognitive decline in mitochondrial previous termdisorders.next term	topic_bd
75668	1	355259	7	NULL	NULL	0	NULL	Schizophrenia	MedicalFinding	phenotype of	share with					BPD-I	MedicalFinding	phenotype of			NULL		0	NULL	NULL	NULL	NULL	NULL	Schizophrenia and BPD-I share many overlapping phenotypes ([Lin and Mitchell, 2008] and [Thaker, 2008]). Evidence for shared genetic factors derives from pharmacology, pathology, family studies and DNA linkage analysis 	topic_bd
75669	1	355260	7	NULL	NULL	0	NULL	mtDNA	NucleicAcid	mutation of	 cause					mitochondrial disorders	MedicalFinding	primary disease in			NULL		0	NULL	NULL	NULL	NULL	NULL	the primary disease-causing event in mitochondrial disorders is the mtDNA mutation.	topic_bd
75670	1	355261	7	NULL	NULL	0	NULL	mitochondrial diseases	MedicalFinding		comorbid with					psychotic symptoms	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely, bona fide mitochondrial diseases are frequently comorbid with psychotic symptoms and misdiagnosed as SZ or BPD	topic_bd
75671	2	355261	7	NULL	NULL	0	NULL	mitochondrial diseases	MedicalFinding		misdiagnosed as					SZ	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely, bona fide mitochondrial diseases are frequently comorbid with psychotic symptoms and misdiagnosed as SZ or BPD	topic_bd
75672	3	355261	7	NULL	NULL	0	NULL	mitochondrial diseases	MedicalFinding		misdiagnosed as					BPD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely, bona fide mitochondrial diseases are frequently comorbid with psychotic symptoms and misdiagnosed as SZ or BPD	topic_bd
75673	1	355262	7	NULL	NULL	0	NULL	Mood stabilizers	Chemical		protect against		partial			mitochondrial toxicity	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Mood stabilizers provide partial protection against mitochondrial toxicity, whereas first-generation antipsychotic drugs might have adverse effects on mitochondrial respiration	topic_bd
75674	2	355262	7	NULL	NULL	0	NULL	antipsychotic drugs	Chemical		adverse effects on					mitochondrial respiration	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Mood stabilizers provide partial protection against mitochondrial toxicity, whereas first-generation antipsychotic drugs might have adverse effects on mitochondrial respiration	topic_bd
75675	1	355263	7	NULL	NULL	NULL	NULL	Mitochondrial pathology	MedicalFinding		consequence of		could be			genetic susceptibility	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mitochondrial pathology could be the consequence of genetic susceptibility secondary to dysregulation of other neurotransmitter systems 	topic_bd
75676	2	355263	7	NULL	NULL	NULL	NULL	statement 1	Process		secondary to					neurotransmitter system	Chemical	dysregulation of 			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mitochondrial pathology could be the consequence of genetic susceptibility secondary to dysregulation of other neurotransmitter systems 	topic_bd
75677	1	355264	7	NULL	NULL	0	NULL	Mitochondrial pathology	MedicalFinding		consequence of		could be			genetic susceptibility	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial pathology could be the consequence of genetic susceptibility secondary to dysregulation of other neurotransmitter systems or the results of environmental impacts such as exposure to toxins, famine, infections and substance abuse all of which are known risk factors for BPD and SZ.	topic_bd
75678	2	355264	7	NULL	NULL	0	NULL	statement 1	Process		secondary to					neurotransmitter system	Chemical	dysregulation of 			NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial pathology could be the consequence of genetic susceptibility secondary to dysregulation of other neurotransmitter systems or the results of environmental impacts such as exposure to toxins, famine, infections and substance abuse all of which are known risk factors for BPD and SZ.	topic_bd
75679	3	355264	7	NULL	NULL	0	NULL	 toxins	Chemical	exposure to	risk factor of					BPD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial pathology could be the consequence of genetic susceptibility secondary to dysregulation of other neurotransmitter systems or the results of environmental impacts such as exposure to toxins, famine, infections and substance abuse all of which are known risk factors for BPD and SZ.	topic_bd
75680	4	355264	7	NULL	NULL	0	NULL	famine	PhysicalPhenomenon		risk factor of					BPD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial pathology could be the consequence of genetic susceptibility secondary to dysregulation of other neurotransmitter systems or the results of environmental impacts such as exposure to toxins, famine, infections and substance abuse all of which are known risk factors for BPD and SZ.	topic_bd
75681	5	355264	7	NULL	NULL	0	NULL	infection	MedicalFinding		risk factor of					BPD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial pathology could be the consequence of genetic susceptibility secondary to dysregulation of other neurotransmitter systems or the results of environmental impacts such as exposure to toxins, famine, infections and substance abuse all of which are known risk factors for BPD and SZ.	topic_bd
75682	6	355264	7	NULL	NULL	0	NULL	substance abuse	Chemical		risk factor of					BPD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial pathology could be the consequence of genetic susceptibility secondary to dysregulation of other neurotransmitter systems or the results of environmental impacts such as exposure to toxins, famine, infections and substance abuse all of which are known risk factors for BPD and SZ.	topic_bd
75683	7	355264	7	NULL	NULL	0	NULL	toxins	Chemical	exposure to	risk factor of					SZ	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial pathology could be the consequence of genetic susceptibility secondary to dysregulation of other neurotransmitter systems or the results of environmental impacts such as exposure to toxins, famine, infections and substance abuse all of which are known risk factors for BPD and SZ.	topic_bd
75684	8	355264	7	NULL	NULL	0	NULL	famine	PhysicalPhenomenon		risk factor of					SZ	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial pathology could be the consequence of genetic susceptibility secondary to dysregulation of other neurotransmitter systems or the results of environmental impacts such as exposure to toxins, famine, infections and substance abuse all of which are known risk factors for BPD and SZ.	topic_bd
75685	9	355264	7	NULL	NULL	0	NULL	infection	MedicalFinding		risk factor of					SZ	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial pathology could be the consequence of genetic susceptibility secondary to dysregulation of other neurotransmitter systems or the results of environmental impacts such as exposure to toxins, famine, infections and substance abuse all of which are known risk factors for BPD and SZ.	topic_bd
75686	10	355264	7	NULL	NULL	0	NULL	substance abuse	Chemical		risk factor of					SZ	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial pathology could be the consequence of genetic susceptibility secondary to dysregulation of other neurotransmitter systems or the results of environmental impacts such as exposure to toxins, famine, infections and substance abuse all of which are known risk factors for BPD and SZ.	topic_bd
75687	1	355265	7	NULL	NULL	0	NULL	Mitochondria	CellComponent		smaller in		significantly			PFC	CellComponent				NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondria were significantly smaller in the prefrontal cortex (PFC) of BPD patients compared to normal controls 	topic_bd
75688	2	355265	7	NULL	NULL	0	NULL	statement 1	Process		occur in					BPD	MedicalFinding	patients with			NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondria were significantly smaller in the prefrontal cortex (PFC) of BPD patients compared to normal controls 	topic_bd
75689	3	355265	7	NULL	NULL	0	NULL	PFC	CellComponent		is					prefrontal cortex	CellComponent				NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondria were significantly smaller in the prefrontal cortex (PFC) of BPD patients compared to normal controls 	topic_bd
75690	1	355266	7	NULL	NULL	0	NULL	mitochondria	CellComponent	cellular location of	altered in					lymphoblastoid cell line	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	The cellular location of mitochondria was altered in lymphoblastoid and fibroblast cell lines of BPD patients	topic_bd
75691	2	355266	7	NULL	NULL	NULL	NULL	mitochondria	CellComponent	cellular location of	altered in					 fibroblast cell lines	Cell				NULL		NULL	NULL	NULL	NULL	NULL	NULL	The cellular location of mitochondria was altered in lymphoblastoid and fibroblast cell lines of BPD patients	topic_bd
75692	3	355266	7	NULL	NULL	0	NULL	statement 1	Process		occur in					BPD	MedicalFinding	patients with			NULL		0	NULL	NULL	NULL	NULL	NULL	The cellular location of mitochondria was altered in lymphoblastoid and fibroblast cell lines of BPD patients	topic_bd
75693	4	355266	7	NULL	NULL	0	NULL	statement 2	Process		occur in					BPD	MedicalFinding	patients with			NULL		0	NULL	NULL	NULL	NULL	NULL	The cellular location of mitochondria was altered in lymphoblastoid and fibroblast cell lines of BPD patients	topic_bd
75694	1	355267	7	NULL	NULL	NULL	NULL	BPD	MedicalFinding	lymphocytes of patients of	does not respond to 					glucose	Chemical	deprivation of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Lymphocytes of BPD patients failed to respond to glucose deprivation while lymphocytes of normal controls responded with an upregulation of the elements of the electron transport chain	topic_bd
75695	2	355267	7	NULL	NULL	0	NULL	normal lymphocytes	cell		respond to					glucose 	Chemical	deprivation of			NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocytes of BPD patients failed to respond to glucose deprivation while lymphocytes of normal controls responded with an upregulation of the elements of the electron transport chain	topic_bd
75696	3	355267	7	NULL	NULL	0	NULL	statement 2	Process		upregulate					electron transport chain	Process	elements of			NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocytes of BPD patients failed to respond to glucose deprivation while lymphocytes of normal controls responded with an upregulation of the elements of the electron transport chain	topic_bd
74595	1	355271	6	NULL	NULL	0	NULL	SERM	Chemical		act on					estrogen receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Selective Estrogen Receptor Modulators (SERMs) are a class of compounds that act on the estrogen receptor.	topic_bc
74596	1	355272	6	NULL	NULL	NULL	NULL	raloxifene hydrochloride	Chemical		reduces					breast cancer	MedicalFinding	risk of;; invasive			NULL	post-menopausal women with Osteoporosis	NULL	NULL	NULL	NULL	NULL	NULL	On September 13, 2007, the U. S. Food and Drug Administration approved raloxifene hydrochloride tablets (Evista® tablets, made by Eli Lilly and Company) for reduction in the risk of invasive breast cancer in postmenopausal women with osteoporosis and in postmenopausal women at high risk for invasive breast cancer.	topic_bc
74607	2	355272	6	NULL	NULL	0	NULL	post-menopausal women	Person		is at					breast cancer	MedicalFinding	high risk;; invasive			NULL		0	NULL	NULL	NULL	NULL	NULL	On September 13, 2007, the U. S. Food and Drug Administration approved raloxifene hydrochloride tablets (Evista® tablets, made by Eli Lilly and Company) for reduction in the risk of invasive breast cancer in postmenopausal women with osteoporosis and in postmenopausal women at high risk for invasive breast cancer.	topic_bc
74608	3	355272	6	NULL	NULL	0	NULL	raloxifene hydrochloride	Chemical		reduces					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	On September 13, 2007, the U. S. Food and Drug Administration approved raloxifene hydrochloride tablets (Evista® tablets, made by Eli Lilly and Company) for reduction in the risk of invasive breast cancer in postmenopausal women with osteoporosis and in postmenopausal women at high risk for invasive breast cancer.	topic_bc
74382	1	355273	5	NULL	NULL	0	NULL	Asenapine	Chemical		is a type of					atypical antipsychotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Asenapine is an atypical antipsychotic approved by the US Food and Drug Administration in adults for treatment of schizophrenia or acute treatment, as monotherapy or adjunct therapy to lithium or valproate, of manic or mixed episodes of bipolar I disorder.	topic_sch
74383	2	355273	5	NULL	NULL	0	NULL	Asenapine	Chemical		is approved by					US Food and Drug Administration	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Asenapine is an atypical antipsychotic approved by the US Food and Drug Administration in adults for treatment of schizophrenia or acute treatment, as monotherapy or adjunct therapy to lithium or valproate, of manic or mixed episodes of bipolar I disorder.	topic_sch
74384	3	355273	5	NULL	NULL	0	NULL	Asenapine	Chemical		treats					schizophrenia	MedicalFinding				NULL	adults	0	NULL	NULL	NULL	NULL	NULL	Asenapine is an atypical antipsychotic approved by the US Food and Drug Administration in adults for treatment of schizophrenia or acute treatment, as monotherapy or adjunct therapy to lithium or valproate, of manic or mixed episodes of bipolar I disorder.	topic_sch
74385	4	355273	5	NULL	NULL	0	NULL	Lithium	Chemical		treats					bipolar I disorder	MedicalFinding	 manic episodes of;;mixed episodes of			NULL		0	NULL	NULL	NULL	NULL	NULL	Asenapine is an atypical antipsychotic approved by the US Food and Drug Administration in adults for treatment of schizophrenia or acute treatment, as monotherapy or adjunct therapy to lithium or valproate, of manic or mixed episodes of bipolar I disorder.	topic_sch
74386	5	355273	5	NULL	NULL	0	NULL	valproate	Chemical		treats					bipolar I disorder	MedicalFinding	manic episodes of;;mixed episodes of			NULL		0	NULL	NULL	NULL	NULL	NULL	Asenapine is an atypical antipsychotic approved by the US Food and Drug Administration in adults for treatment of schizophrenia or acute treatment, as monotherapy or adjunct therapy to lithium or valproate, of manic or mixed episodes of bipolar I disorder.	topic_sch
74387	6	355273	5	NULL	NULL	0	NULL	Asenapine	Chemical		is an adjunct therapy to					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Asenapine is an atypical antipsychotic approved by the US Food and Drug Administration in adults for treatment of schizophrenia or acute treatment, as monotherapy or adjunct therapy to lithium or valproate, of manic or mixed episodes of bipolar I disorder.	topic_sch
74388	7	355273	5	NULL	NULL	0	NULL	Asenapine	Chemical		is an adjunct therapy to					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Asenapine is an atypical antipsychotic approved by the US Food and Drug Administration in adults for treatment of schizophrenia or acute treatment, as monotherapy or adjunct therapy to lithium or valproate, of manic or mixed episodes of bipolar I disorder.	topic_sch
74389	1	355275	5	NULL	NULL	0	NULL	major histocompatability complex	GP		is present in					chromosome 6p	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	The major histocompatability complex on chromosome 6p has often been identified as containing potential risk factors for schizophrenia.	topic_sch
74390	2	355275	5	NULL	NULL	0	NULL	major histocompatability complex	GP		plays a role in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The major histocompatability complex on chromosome 6p has often been identified as containing potential risk factors for schizophrenia.	topic_sch
74391	1	355276	5	NULL	NULL	0	NULL	NOTCH4 gene	GP		is located in					6p21.3	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	The NOTCH4 gene is located within this region (6p21.3) and sequence variants have previously shown association to the disease.	topic_sch
74392	1	355277	5	NULL	NULL	0	NULL	 NOTCH4 gene	GP		is located in					6p21.3	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	The NOTCH4 gene is located within this region (6p21.3) and sequence variants have previously shown association to the disease. It is further implicated from a functional standpoint as it plays a critical role during the neurodevelopmental process.	topic_sch
74393	2	355277	5	NULL	NULL	0	NULL	 NOTCH4 gene	GP		plays a role in					neurodevelopment	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The NOTCH4 gene is located within this region (6p21.3) and sequence variants have previously shown association to the disease. It is further implicated from a functional standpoint as it plays a critical role during the neurodevelopmental process.	topic_sch
74394	1	355278	5	NULL	NULL	0	NULL	25 C/T polymorphism	Process		is not associated with					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	It also established that the -25 C/T polymorphism was not associated to schizophrenia.	topic_sch
74395	1	355279	5	NULL	NULL	0	NULL	autism	MedicalFinding		is a type of					PDDs	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The term pervasive developmental disorders (PDDs) refers to a group of developmental conditions that involve delayed or impaired communication and social skills, behaviors, and cognitive skills (learning). autism is the best-known of the PDDs	topic_aut
74396	2	355279	5	NULL	NULL	0	NULL	PDDs	MedicalFinding		is					pervasive developmental disorders	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The term pervasive developmental disorders (PDDs) refers to a group of developmental conditions that involve delayed or impaired communication and social skills, behaviors, and cognitive skills (learning). autism is the best-known of the PDDs	topic_aut
74397	3	355279	5	NULL	NULL	0	NULL	PDDs	MedicalFinding		involves					communication	AbstractConcept	delayed			NULL		0	NULL	NULL	NULL	NULL	NULL	The term pervasive developmental disorders (PDDs) refers to a group of developmental conditions that involve delayed or impaired communication and social skills, behaviors, and cognitive skills (learning). autism is the best-known of the PDDs	topic_aut
74398	4	355279	5	NULL	NULL	0	NULL	PDDs	MedicalFinding		involves					communication	AbstractConcept	impaired			NULL		0	NULL	NULL	NULL	NULL	NULL	The term pervasive developmental disorders (PDDs) refers to a group of developmental conditions that involve delayed or impaired communication and social skills, behaviors, and cognitive skills (learning). autism is the best-known of the PDDs	topic_aut
74399	5	355279	5	NULL	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The term pervasive developmental disorders (PDDs) refers to a group of developmental conditions that involve delayed or impaired communication and social skills, behaviors, and cognitive skills (learning). autism is the best-known of the PDDs	topic_aut
74400	6	355279	5	NULL	NULL	0	NULL	PDDs	MedicalFinding		involves					social skills	AbstractConcept	delayed			NULL		0	NULL	NULL	NULL	NULL	NULL	The term pervasive developmental disorders (PDDs) refers to a group of developmental conditions that involve delayed or impaired communication and social skills, behaviors, and cognitive skills (learning). autism is the best-known of the PDDs	topic_aut
74401	7	355279	5	NULL	NULL	0	NULL	PDDs	MedicalFinding		involves					social skills	AbstractConcept	impaired			NULL		0	NULL	NULL	NULL	NULL	NULL	The term pervasive developmental disorders (PDDs) refers to a group of developmental conditions that involve delayed or impaired communication and social skills, behaviors, and cognitive skills (learning). autism is the best-known of the PDDs	topic_aut
74402	8	355279	5	NULL	NULL	0	NULL	statement 6	Process		is an alternative to					statement 7	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The term pervasive developmental disorders (PDDs) refers to a group of developmental conditions that involve delayed or impaired communication and social skills, behaviors, and cognitive skills (learning). autism is the best-known of the PDDs	topic_aut
74403	9	355279	5	NULL	NULL	0	NULL	PDDs	MedicalFinding		involves					behavior	AbstractConcept	delayed			NULL		0	NULL	NULL	NULL	NULL	NULL	The term pervasive developmental disorders (PDDs) refers to a group of developmental conditions that involve delayed or impaired communication and social skills, behaviors, and cognitive skills (learning). autism is the best-known of the PDDs	topic_aut
74404	10	355279	5	NULL	NULL	0	NULL	PDDs	MedicalFinding		involves					behavior	AbstractConcept	impaired			NULL		0	NULL	NULL	NULL	NULL	NULL	The term pervasive developmental disorders (PDDs) refers to a group of developmental conditions that involve delayed or impaired communication and social skills, behaviors, and cognitive skills (learning). autism is the best-known of the PDDs	topic_aut
74405	11	355279	5	NULL	NULL	0	NULL	statement 9	Process		is an alternative to					statement 10	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The term pervasive developmental disorders (PDDs) refers to a group of developmental conditions that involve delayed or impaired communication and social skills, behaviors, and cognitive skills (learning). autism is the best-known of the PDDs	topic_aut
74406	12	355279	5	NULL	NULL	0	NULL	PDDs	MedicalFinding		involves					cognitive skills	MentalProcess	delayed			NULL		0	NULL	NULL	NULL	NULL	NULL	The term pervasive developmental disorders (PDDs) refers to a group of developmental conditions that involve delayed or impaired communication and social skills, behaviors, and cognitive skills (learning). autism is the best-known of the PDDs	topic_aut
74407	13	355279	5	NULL	NULL	0	NULL	PDDs	MedicalFinding		involves					cognitive skills	MentalProcess	impaired			NULL		0	NULL	NULL	NULL	NULL	NULL	The term pervasive developmental disorders (PDDs) refers to a group of developmental conditions that involve delayed or impaired communication and social skills, behaviors, and cognitive skills (learning). autism is the best-known of the PDDs	topic_aut
74408	14	355279	5	NULL	NULL	0	NULL	statement 12	Process		is an alternative to					statement 13	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The term pervasive developmental disorders (PDDs) refers to a group of developmental conditions that involve delayed or impaired communication and social skills, behaviors, and cognitive skills (learning). autism is the best-known of the PDDs	topic_aut
75697	1	355280	7	NULL	NULL	0	NULL	VPA	Chemical		is metabolized in					mitochondria	CellComponent				NULL		0	NULL	NULL	NULL	NULL	NULL	The mood stabilizer VPA is metabolized in mitochondria, and many antipsychotic drugs or their metabolites are taken up into mitochondria	topic_bd
75698	2	355280	7	NULL	NULL	0	NULL	antipsychotic drugs	Chemical		taken up in					mitochondria	CellComponent				NULL		0	NULL	NULL	NULL	NULL	NULL	The mood stabilizer VPA is metabolized in mitochondria, and many antipsychotic drugs or their metabolites are taken up into mitochondria	topic_bd
75699	3	355280	7	NULL	NULL	0	NULL	antipsychotic drugs	Chemical	metabolites of	taken up in					mitochondria	CellComponent				NULL		0	NULL	NULL	NULL	NULL	NULL	The mood stabilizer VPA is metabolized in mitochondria, and many antipsychotic drugs or their metabolites are taken up into mitochondria	topic_bd
75705	4	355280	7	NULL	NULL	0	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The mood stabilizer VPA is metabolized in mitochondria, and many antipsychotic drugs or their metabolites are taken up into mitochondria	topic_bd
75700	1	355281	7	NULL	NULL	0	NULL	VPA	Chemical		is metabolized in					mitochondria	CellComponent				NULL		0	NULL	NULL	NULL	NULL	NULL	The mood stabilizer VPA is metabolized in mitochondria, and many antipsychotic drugs or their metabolites are taken up into mitochondria 	topic_bd
75701	2	355281	7	NULL	NULL	0	NULL	VPA	Chemical		is a type of					mood stabilizer	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The mood stabilizer VPA is metabolized in mitochondria, and many antipsychotic drugs or their metabolites are taken up into mitochondria 	topic_bd
75702	3	355281	7	NULL	NULL	0	NULL	antipsychotic drugs	Chemical		taken up in					mitochondria	CellComponent				NULL		0	NULL	NULL	NULL	NULL	NULL	The mood stabilizer VPA is metabolized in mitochondria, and many antipsychotic drugs or their metabolites are taken up into mitochondria 	topic_bd
75703	4	355281	7	NULL	NULL	0	NULL	antipsychotic drugs	Chemical	metabolites of	taken up in					mitochondria	CellComponent				NULL		0	NULL	NULL	NULL	NULL	NULL	The mood stabilizer VPA is metabolized in mitochondria, and many antipsychotic drugs or their metabolites are taken up into mitochondria 	topic_bd
75704	5	355281	7	NULL	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The mood stabilizer VPA is metabolized in mitochondria, and many antipsychotic drugs or their metabolites are taken up into mitochondria 	topic_bd
75706	1	355282	7	NULL	NULL	0	NULL	VPA	Chemical		increase					 oxygen consumption	Process	mitochondrial			NULL		0	NULL	NULL	NULL	NULL	NULL	VPA and lithium induced increases in mitochondrial oxygen consumption and mitochondrial membrane potential	topic_bd
75707	2	355282	7	NULL	NULL	0	NULL	VPA	Chemical		increase					membrane potential	QuantityOrMeasure	mitochondrial			NULL		0	NULL	NULL	NULL	NULL	NULL	VPA and lithium induced increases in mitochondrial oxygen consumption and mitochondrial membrane potential	topic_bd
75708	3	355282	7	NULL	NULL	0	NULL	lithium	Chemical		increase					oxygen consumption	Process	mitochondrial			NULL		0	NULL	NULL	NULL	NULL	NULL	VPA and lithium induced increases in mitochondrial oxygen consumption and mitochondrial membrane potential	topic_bd
75709	4	355282	7	NULL	NULL	0	NULL	lithium	Chemical		increase					membrane potential	QuantityOrMeasure	mitochondrial			NULL		0	NULL	NULL	NULL	NULL	NULL	VPA and lithium induced increases in mitochondrial oxygen consumption and mitochondrial membrane potential	topic_bd
75710	1	355283	7	NULL	NULL	0	NULL	 mood stabilizers	Chemical		alleviate					BPD	MedicalFinding	symptoms of			NULL		0	NULL	NULL	NULL	NULL	NULL	This indicates that mood stabilizers may alleviate some of the symptoms of BPD by improving mitochondrial function	topic_bd
75711	2	355283	7	NULL	NULL	0	NULL	statement 1	Process		improve					mitochondrial function	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	This indicates that mood stabilizers may alleviate some of the symptoms of BPD by improving mitochondrial function	topic_bd
75712	1	355284	7	NULL	NULL	0	NULL	lithium	Chemical		shows					antiapoptotic effects	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Both drugs [lithium and VPA] also have antiapoptotic effects. They are known to inhibit cytochrome c release from mitochondria and to increase expression of the anti-apoptotic gene Bcl-2.	topic_bd
75713	2	355284	7	NULL	NULL	0	NULL	VPA	Chemical		shows					antiapoptotic effects	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Both drugs [lithium and VPA] also have antiapoptotic effects. They are known to inhibit cytochrome c release from mitochondria and to increase expression of the anti-apoptotic gene Bcl-2.	topic_bd
75714	3	355284	7	NULL	NULL	0	NULL	lithium	Chemical		inhibit					cytochrome c	GP	release of			NULL		0	NULL	NULL	NULL	NULL	NULL	Both drugs [lithium and VPA] also have antiapoptotic effects. They are known to inhibit cytochrome c release from mitochondria and to increase expression of the anti-apoptotic gene Bcl-2.	topic_bd
75715	4	355284	7	NULL	NULL	0	NULL	statement 3	Process		occur from					mitochondria	CellComponent				NULL		0	NULL	NULL	NULL	NULL	NULL	Both drugs [lithium and VPA] also have antiapoptotic effects. They are known to inhibit cytochrome c release from mitochondria and to increase expression of the anti-apoptotic gene Bcl-2.	topic_bd
75716	5	355284	7	NULL	NULL	0	NULL	lithium	Chemical		increase					Bcl-2	GP	expression of			NULL		0	NULL	NULL	NULL	NULL	NULL	Both drugs [lithium and VPA] also have antiapoptotic effects. They are known to inhibit cytochrome c release from mitochondria and to increase expression of the anti-apoptotic gene Bcl-2.	topic_bd
75717	6	355284	7	NULL	NULL	0	NULL	Bcl-2	GP		is a type of					anti-apoptotic gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Both drugs [lithium and VPA] also have antiapoptotic effects. They are known to inhibit cytochrome c release from mitochondria and to increase expression of the anti-apoptotic gene Bcl-2.	topic_bd
75718	7	355284	7	NULL	NULL	0	NULL	VPA	Chemical		inhibit					cytochrome c	GP	release of			NULL		0	NULL	NULL	NULL	NULL	NULL	Both drugs [lithium and VPA] also have antiapoptotic effects. They are known to inhibit cytochrome c release from mitochondria and to increase expression of the anti-apoptotic gene Bcl-2.	topic_bd
75719	8	355284	7	NULL	NULL	0	NULL	statement 7	Process		occur from					mitochondria	CellComponent				NULL		0	NULL	NULL	NULL	NULL	NULL	Both drugs [lithium and VPA] also have antiapoptotic effects. They are known to inhibit cytochrome c release from mitochondria and to increase expression of the anti-apoptotic gene Bcl-2.	topic_bd
75720	9	355284	7	NULL	NULL	0	NULL	VPA	Chemical		increase					Bcl-2	GP	expression of			NULL		0	NULL	NULL	NULL	NULL	NULL	Both drugs [lithium and VPA] also have antiapoptotic effects. They are known to inhibit cytochrome c release from mitochondria and to increase expression of the anti-apoptotic gene Bcl-2.	topic_bd
75721	1	355286	7	NULL	NULL	0	NULL	VPA	Chemical		is a inhibitor of					histone deacetylase	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	VPA is a histone deacetylase inhibitor and facilitates gene expression via this epigenetic mechanism	topic_bd
75722	2	355286	7	NULL	NULL	0	NULL	VPA	Chemical		facilitate					gene expression	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	VPA is a histone deacetylase inhibitor and facilitates gene expression via this epigenetic mechanism	topic_bd
75723	3	355286	7	NULL	NULL	0	NULL	statement 2	Process		occur via					epigenetic mechanism	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	VPA is a histone deacetylase inhibitor and facilitates gene expression via this epigenetic mechanism	topic_bd
75724	1	355287	7	NULL	NULL	0	NULL	conventional antipsychotics	Chemical		inhibitors of					dopamine D2 receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The first generation of antipsychotic drugs, “conventional antipsychotics”, are potent inhibitors of the dopamine D2 receptor	topic_bd
75725	2	355287	7	NULL	NULL	0	NULL	conventional antipsychotics	Chemical		belongs to					antipsychotic drugs	Chemical	first generation of			NULL		0	NULL	NULL	NULL	NULL	NULL	The first generation of antipsychotic drugs, “conventional antipsychotics”, are potent inhibitors of the dopamine D2 receptor	topic_bd
75726	1	355288	7	NULL	NULL	0	NULL	Atypical antipsychotic drugs	Chemical		target					serotonin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	“Atypical antipsychotic drugs” target other neurotransmitter systems, including serotonin, norepinephrine, and cannabinoids, and produce fewer extrapyramidal side effects	topic_bd
75727	2	355288	7	NULL	NULL	0	NULL	Atypical antipsychotic drugs	Chemical		target					norepinephrine	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	“Atypical antipsychotic drugs” target other neurotransmitter systems, including serotonin, norepinephrine, and cannabinoids, and produce fewer extrapyramidal side effects	topic_bd
75728	3	355288	7	NULL	NULL	0	NULL	Atypical antipsychotic drugs	Chemical		target					cannabinoids	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	“Atypical antipsychotic drugs” target other neurotransmitter systems, including serotonin, norepinephrine, and cannabinoids, and produce fewer extrapyramidal side effects	topic_bd
75729	4	355288	7	NULL	NULL	NULL	NULL	statement 1	Process		produce					extrapyramidal side effects	MedicalFinding	fewer			NULL		NULL	NULL	NULL	NULL	NULL	NULL	“Atypical antipsychotic drugs” target other neurotransmitter systems, including serotonin, norepinephrine, and cannabinoids, and produce fewer extrapyramidal side effects	topic_bd
75730	5	355288	7	NULL	NULL	NULL	NULL	statement 2	Process		produce					extrapyramidal side effects	MedicalFinding	fewer			NULL		NULL	NULL	NULL	NULL	NULL	NULL	“Atypical antipsychotic drugs” target other neurotransmitter systems, including serotonin, norepinephrine, and cannabinoids, and produce fewer extrapyramidal side effects	topic_bd
75731	6	355288	7	NULL	NULL	0	NULL	statement 3	Process		produce					extrapyramidal side effects	MedicalFinding	fewer			NULL		0	NULL	NULL	NULL	NULL	NULL	“Atypical antipsychotic drugs” target other neurotransmitter systems, including serotonin, norepinephrine, and cannabinoids, and produce fewer extrapyramidal side effects	topic_bd
75732	7	355288	7	NULL	NULL	0	NULL	serotonin	Chemical		is a type of					neurotransmitter	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	“Atypical antipsychotic drugs” target other neurotransmitter systems, including serotonin, norepinephrine, and cannabinoids, and produce fewer extrapyramidal side effects	topic_bd
75733	8	355288	7	NULL	NULL	0	NULL	norepinephrine	Chemical		is a type of					neurotransmitter	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	“Atypical antipsychotic drugs” target other neurotransmitter systems, including serotonin, norepinephrine, and cannabinoids, and produce fewer extrapyramidal side effects	topic_bd
75734	9	355288	7	NULL	NULL	0	NULL	cannabinoids	Chemical		is a type of					neurotransmitter	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	“Atypical antipsychotic drugs” target other neurotransmitter systems, including serotonin, norepinephrine, and cannabinoids, and produce fewer extrapyramidal side effects	topic_bd
75735	1	355289	7	NULL	NULL	0	NULL	complex I 	GP	inhibition of	results in					maximal oxygen consumption rate	QuantityOrMeasure	inhibition of			NULL		0	NULL	NULL	NULL	NULL	NULL	Despite the increased complex IV activity seen with many antipsychotics, it appears that their inhibition of complex I results in an overall inhibition of maximal oxygen consumption rate after uncoupling and, more importantly, might reduce the ability to produce ATP. This suggests that antipsychotics might contribute to mitochondrial instability.	topic_bd
75736	2	355289	7	NULL	NULL	0	NULL	statement 1	Process		occur after					uncoupling	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Despite the increased complex IV activity seen with many antipsychotics, it appears that their inhibition of complex I results in an overall inhibition of maximal oxygen consumption rate after uncoupling and, more importantly, might reduce the ability to produce ATP. This suggests that antipsychotics might contribute to mitochondrial instability.	topic_bd
75737	3	355289	7	NULL	NULL	0	NULL	statement 1	Process		reduce		might			ATP	Chemical	ability to produce			NULL		0	NULL	NULL	NULL	NULL	NULL	Despite the increased complex IV activity seen with many antipsychotics, it appears that their inhibition of complex I results in an overall inhibition of maximal oxygen consumption rate after uncoupling and, more importantly, might reduce the ability to produce ATP. This suggests that antipsychotics might contribute to mitochondrial instability.	topic_bd
75738	4	355289	7	NULL	NULL	0	NULL	antipsychotics	Chemical		increase					complex IV activity	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Despite the increased complex IV activity seen with many antipsychotics, it appears that their inhibition of complex I results in an overall inhibition of maximal oxygen consumption rate after uncoupling and, more importantly, might reduce the ability to produce ATP. This suggests that antipsychotics might contribute to mitochondrial instability.	topic_bd
75739	5	355289	7	NULL	NULL	0	NULL	antipsychotics 	Chemical		contribute to		might			mitochondrial instability	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Despite the increased complex IV activity seen with many antipsychotics, it appears that their inhibition of complex I results in an overall inhibition of maximal oxygen consumption rate after uncoupling and, more importantly, might reduce the ability to produce ATP. This suggests that antipsychotics might contribute to mitochondrial instability.	topic_bd
75740	6	355289	7	NULL	NULL	0	NULL	statement 3	Process		suggest					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Despite the increased complex IV activity seen with many antipsychotics, it appears that their inhibition of complex I results in an overall inhibition of maximal oxygen consumption rate after uncoupling and, more importantly, might reduce the ability to produce ATP. This suggests that antipsychotics might contribute to mitochondrial instability.	topic_bd
75741	1	355290	7	NULL	NULL	NULL	NULL	mitochondria	CellComponent	overall stability of 	affected in					BPD	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	A large number of studies have shown that the overall stability of mitochondria, the efficiency of OXPHOS, and the ability to buffer Ca2+ and neutralize ROS, are affected in BPD and SZ. 	topic_bd
75742	2	355290	7	NULL	NULL	0	NULL	mitochondria	CellComponent	overall stability of 	affected in					SZ	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	A large number of studies have shown that the overall stability of mitochondria, the efficiency of OXPHOS, and the ability to buffer Ca2+ and neutralize ROS, are affected in BPD and SZ. 	topic_bd
75743	3	355290	7	NULL	NULL	0	NULL	OXPHOS	Chemical	efficiency of	affected in					BPD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	A large number of studies have shown that the overall stability of mitochondria, the efficiency of OXPHOS, and the ability to buffer Ca2+ and neutralize ROS, are affected in BPD and SZ. 	topic_bd
75744	4	355290	7	NULL	NULL	0	NULL	OXPHOS	Chemical	efficiency of	affected in					SZ	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	A large number of studies have shown that the overall stability of mitochondria, the efficiency of OXPHOS, and the ability to buffer Ca2+ and neutralize ROS, are affected in BPD and SZ. 	topic_bd
75745	5	355290	7	NULL	NULL	0	NULL	Ca2+	Chemical	ability to buffer	affected in					BPD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	A large number of studies have shown that the overall stability of mitochondria, the efficiency of OXPHOS, and the ability to buffer Ca2+ and neutralize ROS, are affected in BPD and SZ. 	topic_bd
75746	6	355290	7	NULL	NULL	0	NULL	Ca2+	Chemical	ability to buffer	affected in					SZ	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	A large number of studies have shown that the overall stability of mitochondria, the efficiency of OXPHOS, and the ability to buffer Ca2+ and neutralize ROS, are affected in BPD and SZ. 	topic_bd
75747	7	355290	7	NULL	NULL	0	NULL	ROS	Chemical	ability to neutralize	affected in					BPD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	A large number of studies have shown that the overall stability of mitochondria, the efficiency of OXPHOS, and the ability to buffer Ca2+ and neutralize ROS, are affected in BPD and SZ. 	topic_bd
75748	8	355290	7	NULL	NULL	0	NULL	ROS	Chemical	ability to neutralize	affected in					SZ	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	A large number of studies have shown that the overall stability of mitochondria, the efficiency of OXPHOS, and the ability to buffer Ca2+ and neutralize ROS, are affected in BPD and SZ. 	topic_bd
75749	1	355291	7	NULL	NULL	NULL	NULL	ROS	Chemical		is a type of					oxygen-containing free radicals	Chemical				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Reactive oxygen species (ROS) are oxygen-containing free radicals created as byproducts of both physiological and abnormal electron transport. 	topic_bd
75750	2	355291	7	NULL	NULL	0	NULL	ROS	Chemical		byproducts of					electron transport	Process	physiological			NULL		0	NULL	NULL	NULL	NULL	NULL	Reactive oxygen species (ROS) are oxygen-containing free radicals created as byproducts of both physiological and abnormal electron transport. 	topic_bd
75751	3	355291	7	NULL	NULL	0	NULL	ROS	Chemical		byproducts of					electron transport	Process	abnormal			NULL		0	NULL	NULL	NULL	NULL	NULL	Reactive oxygen species (ROS) are oxygen-containing free radicals created as byproducts of both physiological and abnormal electron transport. 	topic_bd
75752	4	355291	7	NULL	NULL	0	NULL	ROS	Chemical		is					Reactive oxygen species 	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Reactive oxygen species (ROS) are oxygen-containing free radicals created as byproducts of both physiological and abnormal electron transport. 	topic_bd
75753	1	355293	7	NULL	NULL	NULL	NULL	mitochondrial viability	Process	reduced	decrease					ATP	Chemical	production of;;reserves of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Reduced mitochondrial viability and function causes decreased ATP production and reserves. Ion pumps need ATP to maintain the membrane potential in neurons. Proper information processing depends on the ability of the neuron to maintain a solid membrane potential with minimal leakage. One could imagine how a flaccid membrane potential could lead to (a) diminished information processing, i.e. not all information gets adequately propagated, or (b) chance depolarization leading to an erroneous signal.	topic_bd
75754	2	355293	7	NULL	NULL	NULL	NULL	mitochondrial function	Process	reduced	decrease					ATP	Chemical	production of;;reserves of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Reduced mitochondrial viability and function causes decreased ATP production and reserves. Ion pumps need ATP to maintain the membrane potential in neurons. Proper information processing depends on the ability of the neuron to maintain a solid membrane potential with minimal leakage. One could imagine how a flaccid membrane potential could lead to (a) diminished information processing, i.e. not all information gets adequately propagated, or (b) chance depolarization leading to an erroneous signal.	topic_bd
75755	3	355293	7	NULL	NULL	0	NULL	Ion pumps	CellComponent		need					ATP	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced mitochondrial viability and function causes decreased ATP production and reserves. Ion pumps need ATP to maintain the membrane potential in neurons. Proper information processing depends on the ability of the neuron to maintain a solid membrane potential with minimal leakage. One could imagine how a flaccid membrane potential could lead to (a) diminished information processing, i.e. not all information gets adequately propagated, or (b) chance depolarization leading to an erroneous signal.	topic_bd
75756	4	355293	7	NULL	NULL	NULL	NULL	statement 3	Process		maintain					membrane potential	QuantityOrMeasure				NULL	neurons	NULL	NULL	NULL	NULL	NULL	NULL	Reduced mitochondrial viability and function causes decreased ATP production and reserves. Ion pumps need ATP to maintain the membrane potential in neurons. Proper information processing depends on the ability of the neuron to maintain a solid membrane potential with minimal leakage. One could imagine how a flaccid membrane potential could lead to (a) diminished information processing, i.e. not all information gets adequately propagated, or (b) chance depolarization leading to an erroneous signal.	topic_bd
75757	5	355293	7	NULL	NULL	NULL	NULL	neurons	OrganismPart		maintain					solid membrane potential	QuantityOrMeasure				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Reduced mitochondrial viability and function causes decreased ATP production and reserves. Ion pumps need ATP to maintain the membrane potential in neurons. Proper information processing depends on the ability of the neuron to maintain a solid membrane potential with minimal leakage. One could imagine how a flaccid membrane potential could lead to (a) diminished information processing, i.e. not all information gets adequately propagated, or (b) chance depolarization leading to an erroneous signal.	topic_bd
75758	6	355293	7	NULL	NULL	0	NULL	statement 5	Process		occur with					minimal leakage	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced mitochondrial viability and function causes decreased ATP production and reserves. Ion pumps need ATP to maintain the membrane potential in neurons. Proper information processing depends on the ability of the neuron to maintain a solid membrane potential with minimal leakage. One could imagine how a flaccid membrane potential could lead to (a) diminished information processing, i.e. not all information gets adequately propagated, or (b) chance depolarization leading to an erroneous signal.	topic_bd
75759	7	355293	7	NULL	NULL	NULL	NULL	flaccid membrane potential	QuantityOrMeasure		leads to					diminished information processing	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Reduced mitochondrial viability and function causes decreased ATP production and reserves. Ion pumps need ATP to maintain the membrane potential in neurons. Proper information processing depends on the ability of the neuron to maintain a solid membrane potential with minimal leakage. One could imagine how a flaccid membrane potential could lead to (a) diminished information processing, i.e. not all information gets adequately propagated, or (b) chance depolarization leading to an erroneous signal.	topic_bd
75760	8	355293	7	NULL	NULL	0	NULL	chance depolarization	Process		leads to					erroneous signal	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced mitochondrial viability and function causes decreased ATP production and reserves. Ion pumps need ATP to maintain the membrane potential in neurons. Proper information processing depends on the ability of the neuron to maintain a solid membrane potential with minimal leakage. One could imagine how a flaccid membrane potential could lead to (a) diminished information processing, i.e. not all information gets adequately propagated, or (b) chance depolarization leading to an erroneous signal.	topic_bd
75761	9	355293	7	NULL	NULL	0	NULL	 flaccid membrane potential	QuantityOrMeasure		leads to					statement 8	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced mitochondrial viability and function causes decreased ATP production and reserves. Ion pumps need ATP to maintain the membrane potential in neurons. Proper information processing depends on the ability of the neuron to maintain a solid membrane potential with minimal leakage. One could imagine how a flaccid membrane potential could lead to (a) diminished information processing, i.e. not all information gets adequately propagated, or (b) chance depolarization leading to an erroneous signal.	topic_bd
75762	10	355293	7	NULL	NULL	0	NULL	diminished information processing	Process		is					adequately propagated	Process	not all information gets			NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced mitochondrial viability and function causes decreased ATP production and reserves. Ion pumps need ATP to maintain the membrane potential in neurons. Proper information processing depends on the ability of the neuron to maintain a solid membrane potential with minimal leakage. One could imagine how a flaccid membrane potential could lead to (a) diminished information processing, i.e. not all information gets adequately propagated, or (b) chance depolarization leading to an erroneous signal.	topic_bd
75763	11	355293	7	NULL	NULL	0	NULL	 Proper information processing	Process		depends on					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced mitochondrial viability and function causes decreased ATP production and reserves. Ion pumps need ATP to maintain the membrane potential in neurons. Proper information processing depends on the ability of the neuron to maintain a solid membrane potential with minimal leakage. One could imagine how a flaccid membrane potential could lead to (a) diminished information processing, i.e. not all information gets adequately propagated, or (b) chance depolarization leading to an erroneous signal.	topic_bd
75764	1	355294	7	NULL	NULL	0	NULL	neuronal types 	OrganismPart	energy demands of	responsible for					 vulnerability	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	First, the energy demands of particular neuronal types might be responsible for their vulnerability. For example, in the hippocampus certain populations of GABA interneurons have higher activities of cytochrome c, indicating higher energy demands in these cells (Gulyas et al., 2006). Interestingly, markers for GABA neurons are dramatically reduced in the hippocampus in SZ and BPD (Benes et al., 1998 F.M. Benes, E.W. Kwok, S.L. Vincent and M.S. Todtenkopf, A reduction of nonpyramidal cells in sector CA2 of schizophrenics and manic depressives, Biol. Psychiatry 44 (1998), pp. 88–97. Article | PDF (335 K) | View Record in Scopus | Cited By in Scopus (210)[Benes et al., 1998] and [Heckers et al., 2002]), and in BPD are correlated with a reduction in nuclear genes coding for the mitochondrial electron transport chain (Konradi et al., 2004). Thus, neurons with the highest energy demands are abnormal in BPD and SZ. Other neurons might have lower energy demands and less vulnerability to subtle mitochondrial abnormalities.	topic_bd
75765	2	355294	7	NULL	NULL	0	NULL	GABA interneurons 	OrganismPart		shows					cytochrome c	GP	higher activities of			NULL	 hippocampus	0	NULL	NULL	NULL	NULL	NULL	First, the energy demands of particular neuronal types might be responsible for their vulnerability. For example, in the hippocampus certain populations of GABA interneurons have higher activities of cytochrome c, indicating higher energy demands in these cells (Gulyas et al., 2006). Interestingly, markers for GABA neurons are dramatically reduced in the hippocampus in SZ and BPD (Benes et al., 1998 F.M. Benes, E.W. Kwok, S.L. Vincent and M.S. Todtenkopf, A reduction of nonpyramidal cells in sector CA2 of schizophrenics and manic depressives, Biol. Psychiatry 44 (1998), pp. 88–97. Article | PDF (335 K) | View Record in Scopus | Cited By in Scopus (210)[Benes et al., 1998] and [Heckers et al., 2002]), and in BPD are correlated with a reduction in nuclear genes coding for the mitochondrial electron transport chain (Konradi et al., 2004). Thus, neurons with the highest energy demands are abnormal in BPD and SZ. Other neurons might have lower energy demands and less vulnerability to subtle mitochondrial abnormalities.	topic_bd
75766	3	355294	7	NULL	NULL	0	NULL	statement 2	Process		indicates					hippocampus	OrganismPart	higher energy demands in			NULL		0	NULL	NULL	NULL	NULL	NULL	First, the energy demands of particular neuronal types might be responsible for their vulnerability. For example, in the hippocampus certain populations of GABA interneurons have higher activities of cytochrome c, indicating higher energy demands in these cells (Gulyas et al., 2006). Interestingly, markers for GABA neurons are dramatically reduced in the hippocampus in SZ and BPD (Benes et al., 1998 F.M. Benes, E.W. Kwok, S.L. Vincent and M.S. Todtenkopf, A reduction of nonpyramidal cells in sector CA2 of schizophrenics and manic depressives, Biol. Psychiatry 44 (1998), pp. 88–97. Article | PDF (335 K) | View Record in Scopus | Cited By in Scopus (210)[Benes et al., 1998] and [Heckers et al., 2002]), and in BPD are correlated with a reduction in nuclear genes coding for the mitochondrial electron transport chain (Konradi et al., 2004). Thus, neurons with the highest energy demands are abnormal in BPD and SZ. Other neurons might have lower energy demands and less vulnerability to subtle mitochondrial abnormalities.	topic_bd
75767	4	355294	7	NULL	NULL	NULL	NULL	GABA neurons	OrganismPart		reduced in		dramatically			hippocampus	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	First, the energy demands of particular neuronal types might be responsible for their vulnerability. For example, in the hippocampus certain populations of GABA interneurons have higher activities of cytochrome c, indicating higher energy demands in these cells (Gulyas et al., 2006). Interestingly, markers for GABA neurons are dramatically reduced in the hippocampus in SZ and BPD (Benes et al., 1998 F.M. Benes, E.W. Kwok, S.L. Vincent and M.S. Todtenkopf, A reduction of nonpyramidal cells in sector CA2 of schizophrenics and manic depressives, Biol. Psychiatry 44 (1998), pp. 88–97. Article | PDF (335 K) | View Record in Scopus | Cited By in Scopus (210)[Benes et al., 1998] and [Heckers et al., 2002]), and in BPD are correlated with a reduction in nuclear genes coding for the mitochondrial electron transport chain (Konradi et al., 2004). Thus, neurons with the highest energy demands are abnormal in BPD and SZ. Other neurons might have lower energy demands and less vulnerability to subtle mitochondrial abnormalities.	topic_bd
75768	5	355294	7	NULL	NULL	0	NULL	statement 4	Process		occur in					SZ	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	First, the energy demands of particular neuronal types might be responsible for their vulnerability. For example, in the hippocampus certain populations of GABA interneurons have higher activities of cytochrome c, indicating higher energy demands in these cells (Gulyas et al., 2006). Interestingly, markers for GABA neurons are dramatically reduced in the hippocampus in SZ and BPD (Benes et al., 1998 F.M. Benes, E.W. Kwok, S.L. Vincent and M.S. Todtenkopf, A reduction of nonpyramidal cells in sector CA2 of schizophrenics and manic depressives, Biol. Psychiatry 44 (1998), pp. 88–97. Article | PDF (335 K) | View Record in Scopus | Cited By in Scopus (210)[Benes et al., 1998] and [Heckers et al., 2002]), and in BPD are correlated with a reduction in nuclear genes coding for the mitochondrial electron transport chain (Konradi et al., 2004). Thus, neurons with the highest energy demands are abnormal in BPD and SZ. Other neurons might have lower energy demands and less vulnerability to subtle mitochondrial abnormalities.	topic_bd
75769	6	355294	7	NULL	NULL	0	NULL	statement 4	Process		occur in					BPD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	First, the energy demands of particular neuronal types might be responsible for their vulnerability. For example, in the hippocampus certain populations of GABA interneurons have higher activities of cytochrome c, indicating higher energy demands in these cells (Gulyas et al., 2006). Interestingly, markers for GABA neurons are dramatically reduced in the hippocampus in SZ and BPD (Benes et al., 1998 F.M. Benes, E.W. Kwok, S.L. Vincent and M.S. Todtenkopf, A reduction of nonpyramidal cells in sector CA2 of schizophrenics and manic depressives, Biol. Psychiatry 44 (1998), pp. 88–97. Article | PDF (335 K) | View Record in Scopus | Cited By in Scopus (210)[Benes et al., 1998] and [Heckers et al., 2002]), and in BPD are correlated with a reduction in nuclear genes coding for the mitochondrial electron transport chain (Konradi et al., 2004). Thus, neurons with the highest energy demands are abnormal in BPD and SZ. Other neurons might have lower energy demands and less vulnerability to subtle mitochondrial abnormalities.	topic_bd
75770	7	355294	7	NULL	NULL	0	NULL	nuclear genes	GP		code					electron transport chain	Process	mitochondrial			NULL		0	NULL	NULL	NULL	NULL	NULL	First, the energy demands of particular neuronal types might be responsible for their vulnerability. For example, in the hippocampus certain populations of GABA interneurons have higher activities of cytochrome c, indicating higher energy demands in these cells (Gulyas et al., 2006). Interestingly, markers for GABA neurons are dramatically reduced in the hippocampus in SZ and BPD (Benes et al., 1998 F.M. Benes, E.W. Kwok, S.L. Vincent and M.S. Todtenkopf, A reduction of nonpyramidal cells in sector CA2 of schizophrenics and manic depressives, Biol. Psychiatry 44 (1998), pp. 88–97. Article | PDF (335 K) | View Record in Scopus | Cited By in Scopus (210)[Benes et al., 1998] and [Heckers et al., 2002]), and in BPD are correlated with a reduction in nuclear genes coding for the mitochondrial electron transport chain (Konradi et al., 2004). Thus, neurons with the highest energy demands are abnormal in BPD and SZ. Other neurons might have lower energy demands and less vulnerability to subtle mitochondrial abnormalities.	topic_bd
75771	8	355294	7	NULL	NULL	0	NULL	BPD	MedicalFinding		correlated with					statement 7	Process	reduction in			NULL		0	NULL	NULL	NULL	NULL	NULL	First, the energy demands of particular neuronal types might be responsible for their vulnerability. For example, in the hippocampus certain populations of GABA interneurons have higher activities of cytochrome c, indicating higher energy demands in these cells (Gulyas et al., 2006). Interestingly, markers for GABA neurons are dramatically reduced in the hippocampus in SZ and BPD (Benes et al., 1998 F.M. Benes, E.W. Kwok, S.L. Vincent and M.S. Todtenkopf, A reduction of nonpyramidal cells in sector CA2 of schizophrenics and manic depressives, Biol. Psychiatry 44 (1998), pp. 88–97. Article | PDF (335 K) | View Record in Scopus | Cited By in Scopus (210)[Benes et al., 1998] and [Heckers et al., 2002]), and in BPD are correlated with a reduction in nuclear genes coding for the mitochondrial electron transport chain (Konradi et al., 2004). Thus, neurons with the highest energy demands are abnormal in BPD and SZ. Other neurons might have lower energy demands and less vulnerability to subtle mitochondrial abnormalities.	topic_bd
75772	9	355294	7	NULL	NULL	0	NULL	neurons 	OrganismPart	highest energy demands in	abnormal in					BPD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	First, the energy demands of particular neuronal types might be responsible for their vulnerability. For example, in the hippocampus certain populations of GABA interneurons have higher activities of cytochrome c, indicating higher energy demands in these cells (Gulyas et al., 2006). Interestingly, markers for GABA neurons are dramatically reduced in the hippocampus in SZ and BPD (Benes et al., 1998 F.M. Benes, E.W. Kwok, S.L. Vincent and M.S. Todtenkopf, A reduction of nonpyramidal cells in sector CA2 of schizophrenics and manic depressives, Biol. Psychiatry 44 (1998), pp. 88–97. Article | PDF (335 K) | View Record in Scopus | Cited By in Scopus (210)[Benes et al., 1998] and [Heckers et al., 2002]), and in BPD are correlated with a reduction in nuclear genes coding for the mitochondrial electron transport chain (Konradi et al., 2004). Thus, neurons with the highest energy demands are abnormal in BPD and SZ. Other neurons might have lower energy demands and less vulnerability to subtle mitochondrial abnormalities.	topic_bd
75773	10	355294	7	NULL	NULL	0	NULL	neurons	OrganismPart	highest energy demands in	abnormal in					SZ	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	First, the energy demands of particular neuronal types might be responsible for their vulnerability. For example, in the hippocampus certain populations of GABA interneurons have higher activities of cytochrome c, indicating higher energy demands in these cells (Gulyas et al., 2006). Interestingly, markers for GABA neurons are dramatically reduced in the hippocampus in SZ and BPD (Benes et al., 1998 F.M. Benes, E.W. Kwok, S.L. Vincent and M.S. Todtenkopf, A reduction of nonpyramidal cells in sector CA2 of schizophrenics and manic depressives, Biol. Psychiatry 44 (1998), pp. 88–97. Article | PDF (335 K) | View Record in Scopus | Cited By in Scopus (210)[Benes et al., 1998] and [Heckers et al., 2002]), and in BPD are correlated with a reduction in nuclear genes coding for the mitochondrial electron transport chain (Konradi et al., 2004). Thus, neurons with the highest energy demands are abnormal in BPD and SZ. Other neurons might have lower energy demands and less vulnerability to subtle mitochondrial abnormalities.	topic_bd
74609	1	355301	6	NULL	NULL	NULL	NULL	DES	Chemical		is involved in					breast cancer	MedicalFinding	treatment of 			NULL	post-menopausal women	NULL	NULL	NULL	NULL	NULL	NULL	In 1960, DES was found to be more effective than androgens in the treatment of advanced breast cancer in postmenopausal women.  DES was the hormonal treatment of choice for advanced breast cancer in postmenopausal women until 1977	topic_bc
74610	2	355301	6	NULL	NULL	NULL	NULL	androgens	Chemical		is involved in					breast cancer	MedicalFinding	treatment of			NULL	post-menopausal women	NULL	NULL	NULL	NULL	NULL	NULL	In 1960, DES was found to be more effective than androgens in the treatment of advanced breast cancer in postmenopausal women.  DES was the hormonal treatment of choice for advanced breast cancer in postmenopausal women until 1977	topic_bc
74611	3	355301	6	NULL	NULL	0	NULL	statement 1			is more than					statement 2					NULL		0	NULL	NULL	NULL	NULL	NULL	In 1960, DES was found to be more effective than androgens in the treatment of advanced breast cancer in postmenopausal women.  DES was the hormonal treatment of choice for advanced breast cancer in postmenopausal women until 1977	topic_bc
74612	1	355302	6	NULL	NULL	0	NULL	fibroadenoma patients	GroupOfPeople		have					breast cancer	MedicalFinding	increased risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	patients with fibroadenoma have a slightly higher risk of breast cancer later in life	topic_bc
74613	1	355303	6	NULL	NULL	0	NULL	Sixteen-carbon metabolites	Chemical		are toxic to					cellular DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	 Sixteen-carbon metabolites are also toxic to cellular DNA. Synthetic xenoestrogens apparently block the 2-carbon pathway and promote 16-carbon metabolism	topic_bc
74614	2	355303	6	NULL	NULL	0	NULL	xenoestrogens	Chemical		block					2-carbon pathway 	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	 Sixteen-carbon metabolites are also toxic to cellular DNA. Synthetic xenoestrogens apparently block the 2-carbon pathway and promote 16-carbon metabolism	topic_bc
74615	3	355303	6	NULL	NULL	0	NULL	xenoestrogens	Chemical		promote					16-carbon metabolism	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 Sixteen-carbon metabolites are also toxic to cellular DNA. Synthetic xenoestrogens apparently block the 2-carbon pathway and promote 16-carbon metabolism	topic_bc
74645	1	355304	6	NULL	NULL	NULL	NULL	Bras			obstruct					lymph	CellComponent	flow of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	have suggested that bras cause breast cancer by obstructing lymph flow	topic_bc
74646	2	355304	6	NULL	NULL	0	NULL	statement 1	Process		leads to					breast cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	have suggested that bras cause breast cancer by obstructing lymph flow	topic_bc
74648	1	355305	6	NULL	NULL	0	NULL	alcohol		use of	is linked to					breast cancer	MedicalFinding	increased risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	The use of alcohol is clearly linked to an increased risk of developing breast cancer.	topic_bc
75571	1	355306	6	NULL	NULL	0	NULL	Premenopausal women	Person		exposed to					smoke	Chemical	secondhand			NULL		0	NULL	NULL	NULL	NULL	NULL	Premenopausal women who are exposed to secondhand smoke on a regular basis have an increased risk of breast cancer	topic_bc
75572	2	355306	6	NULL	NULL	0	NULL	statement 1	Process		increases					breast cancer	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	Premenopausal women who are exposed to secondhand smoke on a regular basis have an increased risk of breast cancer	topic_bc
77450	1	355307	6	NULL	NULL	0	NULL	Honey	Chemical		is abundant in					phenol	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Further, honey samples with richly abundant phenolic content were found to limit oxidant-induced cell death more effectively. Cytotoxic studies of a selected sample on a breast cancer cell displayed growth inhibition, depending on the concentration used	topic_bc
77632	2	355307	6	NULL	NULL	0	NULL	oxidant	Chemical		induces					cell death	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Further, honey samples with richly abundant phenolic content were found to limit oxidant-induced cell death more effectively. Cytotoxic studies of a selected sample on a breast cancer cell displayed growth inhibition, depending on the concentration used	topic_bc
77633	3	355307	6	NULL	NULL	0	NULL	statement 1	Process		inhibits					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Further, honey samples with richly abundant phenolic content were found to limit oxidant-induced cell death more effectively. Cytotoxic studies of a selected sample on a breast cancer cell displayed growth inhibition, depending on the concentration used	topic_bc
75774	1	355308	7	NULL	NULL	0	NULL	alpha-defensin	GP	expression of	enhanced in					colon cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	It is known that alpha-defensin expression is enhanced in colon cancer.	topic_ccc
75775	1	355309	7	NULL	NULL	0	NULL	DEFA 6	GP	expression of	marker for		potential			adenoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the expression of DEFA 6 preferably can be used as a potential diagnostic marker for adenoma and not as a marker for fully blown carcinoma.	topic_ccc
75776	2	355309	7	NULL	NULL	0	NULL	DEFA 6	GP	expression of	not as marker for					fully blown carcinoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the expression of DEFA 6 preferably can be used as a potential diagnostic marker for adenoma and not as a marker for fully blown carcinoma.	topic_ccc
75777	1	355310	7	NULL	NULL	NULL	NULL	DEFA 6	GP	gene expression of	increased in		moderately			tumor samples	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	The median gene expression of human defensin alpha 6 (DEFA 6) has been found to be moderately increased (~ 5 fold) in tumor samples derived from individuals with colorectal cancer (CRC) when compared to their normal counterparts.	topic_ccc
75778	2	355310	7	NULL	NULL	0	NULL	statement 1	Process		occur in					CRC	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The median gene expression of human defensin alpha 6 (DEFA 6) has been found to be moderately increased (~ 5 fold) in tumor samples derived from individuals with colorectal cancer (CRC) when compared to their normal counterparts.	topic_ccc
75779	3	355310	7	NULL	NULL	0	NULL	CRC	MedicalFinding		is					colorectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The median gene expression of human defensin alpha 6 (DEFA 6) has been found to be moderately increased (~ 5 fold) in tumor samples derived from individuals with colorectal cancer (CRC) when compared to their normal counterparts.	topic_ccc
75780	4	355310	7	NULL	NULL	0	NULL	DEFA 6	GP		is					human defensin alpha 6 	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The median gene expression of human defensin alpha 6 (DEFA 6) has been found to be moderately increased (~ 5 fold) in tumor samples derived from individuals with colorectal cancer (CRC) when compared to their normal counterparts.	topic_ccc
75781	1	355311	7	NULL	NULL	0	NULL	IGFBP-rP1	GP		expressed in		strongly			low grade colorectal carcinoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	 IGFBP-rP1 strongly expressed in low grade colorectal carcinoma and weakly expressed in high grade colorectal carcinoma. 	topic_ccc
75782	2	355311	7	NULL	NULL	0	NULL	IGFBP-rP1	GP		expressed in		weakly			high grade colorectal carcinoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	 IGFBP-rP1 strongly expressed in low grade colorectal carcinoma and weakly expressed in high grade colorectal carcinoma. 	topic_ccc
75783	1	355312	7	NULL	NULL	0	NULL	IGFBP-rP1	GP		upregulate					TAGLN	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 IGFBP-rP1 could upregulate Transgelin (TAGLN)	topic_ccc
75784	2	355312	7	NULL	NULL	0	NULL	TAGLN	GP		is					Transgelin 	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 IGFBP-rP1 could upregulate Transgelin (TAGLN)	topic_ccc
75785	1	355313	7	NULL	NULL	0	NULL	IGFBP-rP1	GP		upregulate					TAGLN	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY	topic_ccc
75786	2	355313	7	NULL	NULL	0	NULL	TAGLN	GP		is involved in					Transgelin	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY	topic_ccc
75787	3	355313	7	NULL	NULL	0	NULL	IGFBP-rP1	GP		downregulate					SRY	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY	topic_ccc
75788	1	355314	7	NULL	NULL	0	NULL	IGFBP-rP1	GP		upregulate					TAGLN	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1)	topic_ccc
75789	2	355314	7	NULL	NULL	0	NULL	IGFBP-rP1	GP		downregulate					SRY-box9	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1)	topic_ccc
75790	3	355314	7	NULL	NULL	0	NULL	IGFBP-rP1	GP		downregulate					SOX9	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1)	topic_ccc
75791	4	355314	7	NULL	NULL	0	NULL	IGFBP-rP1	GP		downregulate					IRS1	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1)	topic_ccc
75792	5	355314	7	NULL	NULL	0	NULL	TAGLN	GP		is					Transgelin	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1)	topic_ccc
75793	6	355314	7	NULL	NULL	0	NULL	SRY	GP		is					sex determining region Y	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1)	topic_ccc
75794	7	355314	7	NULL	NULL	0	NULL	IRS1	GP		is					insulin receptor substrate 1	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1)	topic_ccc
75795	1	355315	7	NULL	NULL	0	NULL	IGFBP-rP1	GP		upregulate					TAGLN	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B),	topic_ccc
75796	2	355315	7	NULL	NULL	0	NULL	IGFBP-rP1	GP		downregulate					SRY-box 9	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B),	topic_ccc
75797	3	355315	7	NULL	NULL	0	NULL	IGFBP-rP1 	GP		downregulate					IRS1	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B),	topic_ccc
75798	4	355315	7	NULL	NULL	0	NULL	IGFBP-rP1	GP		downregulate					CDKN2B	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B),	topic_ccc
75799	5	355315	7	NULL	NULL	0	NULL	p15	GP		inhibits					CDK4	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B),	topic_ccc
75800	6	355315	7	NULL	NULL	0	NULL	IGFBP-rP1	GP		downregulate					SOX9	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B),	topic_ccc
75801	7	355315	7	NULL	NULL	0	NULL	TAGLN	GP		is					Transgelin	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B),	topic_ccc
75802	8	355315	7	NULL	NULL	0	NULL	IRS1	GP		is					 insulin receptor substrate 1	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B),	topic_ccc
75803	9	355315	7	NULL	NULL	0	NULL	CDKN2B	GP		is					cyclin-dependent kinase inhibitor 2B	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B),	topic_ccc
75804	10	355315	7	NULL	NULL	0	NULL	SRY	GP		is					sex determining region Y	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B),	topic_ccc
75805	1	355316	7	NULL	NULL	0	NULL	IGFBP-rP1	GP		upregulate					TAGLN	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	. IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B), amphiregulin(schwannoma-derived growth factor) (AREG)	topic_ccc
75806	2	355316	7	NULL	NULL	0	NULL	IGFBP-rP1	GP		downregulate					SRY-box 9	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	. IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B), amphiregulin(schwannoma-derived growth factor) (AREG)	topic_ccc
75807	3	355316	7	NULL	NULL	0	NULL	IGFBP-rP1	GP		downregulate					SOX9	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	. IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B), amphiregulin(schwannoma-derived growth factor) (AREG)	topic_ccc
75808	4	355316	7	NULL	NULL	0	NULL	IGFBP-rP1	GP		downregulate					IRS1	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	. IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B), amphiregulin(schwannoma-derived growth factor) (AREG)	topic_ccc
75809	5	355316	7	NULL	NULL	0	NULL	IGFBP-rP1 	GP		downregulate					CDKN2B	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	. IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B), amphiregulin(schwannoma-derived growth factor) (AREG)	topic_ccc
75810	6	355316	7	NULL	NULL	0	NULL	IGFBP-rP1	GP		downregulate					AREG	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	. IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B), amphiregulin(schwannoma-derived growth factor) (AREG)	topic_ccc
75811	7	355316	7	NULL	NULL	0	NULL	TAGLN	GP		is					Transgelin	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	. IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B), amphiregulin(schwannoma-derived growth factor) (AREG)	topic_ccc
75812	8	355316	7	NULL	NULL	0	NULL	SRY	GP		is					sex determining region Y	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	. IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B), amphiregulin(schwannoma-derived growth factor) (AREG)	topic_ccc
75813	9	355316	7	NULL	NULL	NULL	NULL	IRS1	GP		is					insulin receptor substrate 1	GP				NULL		NULL	NULL	NULL	NULL	NULL	NULL	. IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B), amphiregulin(schwannoma-derived growth factor) (AREG)	topic_ccc
75814	10	355316	7	NULL	NULL	0	NULL	CDKN2B	GP		is 					cyclin-dependent kinase inhibitor 2B	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	. IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B), amphiregulin(schwannoma-derived growth factor) (AREG)	topic_ccc
75815	11	355316	7	NULL	NULL	0	NULL	p15	GP		inhibit					CDK4	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	. IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B), amphiregulin(schwannoma-derived growth factor) (AREG)	topic_ccc
75816	12	355316	7	NULL	NULL	0	NULL	AREG	GP		is					 amphiregulin	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	. IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B), amphiregulin(schwannoma-derived growth factor) (AREG)	topic_ccc
75817	13	355316	7	NULL	NULL	0	NULL	AREG	GP		is a type of					schwannoma-derived growth factor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	. IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B), amphiregulin(schwannoma-derived growth factor) (AREG)	topic_ccc
75818	1	355317	7	NULL	NULL	0	NULL	IGFBP-rP1	GP		upregulate					TAGLN	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B), amphiregulin(schwannoma-derived growth factor) (AREG) and immediate early response 5-like(IER5L)	topic_ccc
75819	2	355317	7	NULL	NULL	0	NULL	IGFBP-rP1	GP		downregulate					SRY-box 9	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B), amphiregulin(schwannoma-derived growth factor) (AREG) and immediate early response 5-like(IER5L)	topic_ccc
75820	3	355317	7	NULL	NULL	0	NULL	IGFBP-rP1	GP		downregulate					SOX9	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B), amphiregulin(schwannoma-derived growth factor) (AREG) and immediate early response 5-like(IER5L)	topic_ccc
75821	4	355317	7	NULL	NULL	0	NULL	IGFBP-rP1	GP		downregulate					IRS1	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B), amphiregulin(schwannoma-derived growth factor) (AREG) and immediate early response 5-like(IER5L)	topic_ccc
75822	5	355317	7	NULL	NULL	0	NULL	IGFBP-rP1	GP		downregulate					CDKN2B	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B), amphiregulin(schwannoma-derived growth factor) (AREG) and immediate early response 5-like(IER5L)	topic_ccc
75823	6	355317	7	NULL	NULL	0	NULL	IGFBP-rP1	GP		downregulate					AREG	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B), amphiregulin(schwannoma-derived growth factor) (AREG) and immediate early response 5-like(IER5L)	topic_ccc
75824	7	355317	7	NULL	NULL	0	NULL	IGFBP-rP1	GP		downregulate					IER5L	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B), amphiregulin(schwannoma-derived growth factor) (AREG) and immediate early response 5-like(IER5L)	topic_ccc
75825	8	355317	7	NULL	NULL	0	NULL	p15	GP		inhibit					CDK4	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B), amphiregulin(schwannoma-derived growth factor) (AREG) and immediate early response 5-like(IER5L)	topic_ccc
75826	9	355317	7	NULL	NULL	0	NULL	TAGLN	GP		is					Transgelin	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B), amphiregulin(schwannoma-derived growth factor) (AREG) and immediate early response 5-like(IER5L)	topic_ccc
75827	10	355317	7	NULL	NULL	0	NULL	SRY	GP		is involved in					sex determining region Y	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B), amphiregulin(schwannoma-derived growth factor) (AREG) and immediate early response 5-like(IER5L)	topic_ccc
75828	11	355317	7	NULL	NULL	0	NULL	IRS1	GP		is involved in					insulin receptor substrate 1	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B), amphiregulin(schwannoma-derived growth factor) (AREG) and immediate early response 5-like(IER5L)	topic_ccc
75829	12	355317	7	NULL	NULL	0	NULL	CDKN2B	GP		is involved in					cyclin-dependent kinase inhibitor 2B	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B), amphiregulin(schwannoma-derived growth factor) (AREG) and immediate early response 5-like(IER5L)	topic_ccc
75830	13	355317	7	NULL	NULL	0	NULL	AREG	GP		is					amphiregulin	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B), amphiregulin(schwannoma-derived growth factor) (AREG) and immediate early response 5-like(IER5L)	topic_ccc
75831	14	355317	7	NULL	NULL	0	NULL	IER5L	GP		is					immediate early response 5-like	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-rP1 could upreguate Transgelin (TAGLN), downregulate SRY (sex determining region Y)-box 9(campomelic dysplasia, autosomal sex-reversal) (SOX9), insulin receptor substrate 1(IRS1), cyclin-dependent kinase inhibitor 2B (p15, inhibits CDK4) (CDKN2B), amphiregulin(schwannoma-derived growth factor) (AREG) and immediate early response 5-like(IER5L)	topic_ccc
75832	1	355318	7	NULL	NULL	0	NULL	sodium butyrate	Chemical		induce					Caco2 cell	Cell	differentiation of			NULL		0	NULL	NULL	NULL	NULL	NULL	During sodium butyrate-induced Caco2 cell differentiation, IGFBP-rP1 was upregulated 	topic_ccc
75833	1	355319	7	NULL	NULL	0	NULL	IGFBP-rP1	GP	 upregulation of	correlates with					AKP activity	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-rP1 was upregulated and the expression showed significant correlation with the AKP activity	topic_ccc
75834	1	355320	7	NULL	NULL	0	NULL	IGFBP-rP1	GP		associated with					colon cancer	MedicalFinding	differentiation of			NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-rP1 was a potential key molecule associated with colon cancer differentiation. Downregulation of IRS1 and SOX9 may the possible key downstream genes involved in the process.	topic_ccc
75835	2	355320	7	NULL	NULL	0	NULL	IRS1	GP	downregulation of	downstream		possible			gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-rP1 was a potential key molecule associated with colon cancer differentiation. Downregulation of IRS1 and SOX9 may the possible key downstream genes involved in the process.	topic_ccc
75836	3	355320	7	NULL	NULL	0	NULL	SOX9 	GP	downregulation of	downstream		possible			gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-rP1 was a potential key molecule associated with colon cancer differentiation. Downregulation of IRS1 and SOX9 may the possible key downstream genes involved in the process.	topic_ccc
75837	1	355321	7	NULL	NULL	0	NULL	5T4	GP		expressed in					human adenocarcinomas	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The oncofetal antigen, 5T4, is a surface glycoprotein that is expressed on a variety of human adenocarcinomas but rarely on normal tissue. 	topic_ccc
75838	2	355321	7	NULL	NULL	0	NULL	5T4	GP		is a type of					oncofetal antigen	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The oncofetal antigen, 5T4, is a surface glycoprotein that is expressed on a variety of human adenocarcinomas but rarely on normal tissue. 	topic_ccc
75839	3	355321	7	NULL	NULL	0	NULL	5T4	GP		is a type of					surface glycoprotein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The oncofetal antigen, 5T4, is a surface glycoprotein that is expressed on a variety of human adenocarcinomas but rarely on normal tissue. 	topic_ccc
75840	4	355321	7	NULL	NULL	0	NULL	5T4	GP		expressed in		rarely			normal tissue	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	The oncofetal antigen, 5T4, is a surface glycoprotein that is expressed on a variety of human adenocarcinomas but rarely on normal tissue. 	topic_ccc
75841	1	355323	7	NULL	NULL	NULL	NULL	GIV-fl	GP	expression of;;tumor epithelium	correlated with					shortened metastasis-free survival	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	A prospective, exploratory biomarker study conducted on a cohort of 56 patients with stage II colorectal cancer revealed a significant correlation between GIV-fl expression in tumor epithelium and shortened metastasis-free survival.	topic_ccc
75842	2	355323	7	NULL	NULL	0	NULL	statement 1	Process		occur in					stage II colorectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	A prospective, exploratory biomarker study conducted on a cohort of 56 patients with stage II colorectal cancer revealed a significant correlation between GIV-fl expression in tumor epithelium and shortened metastasis-free survival.	topic_ccc
75843	1	355324	7	NULL	NULL	0	NULL	GIV/Girdin	GP	expression of	predicts					patient survival	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of GIV/Girdin, a metastasis-related protein, predicts patient survival in colon cancer.	topic_ccc
75844	2	355324	7	NULL	NULL	0	NULL	statement 1	Process		occur in					colon cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of GIV/Girdin, a metastasis-related protein, predicts patient survival in colon cancer.	topic_ccc
75845	3	355324	7	NULL	NULL	0	NULL	GIV/Girdin	GP		is a type of					metastasis-related protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of GIV/Girdin, a metastasis-related protein, predicts patient survival in colon cancer.	topic_ccc
74409	1	355325	5	NULL	NULL	0	NULL	schizophrenia	OrganismPart		involves					brain	OrganismPart	aberrant topology of;;structural infrastructure of;;network of			NULL		0	NULL	NULL	NULL	NULL	NULL	Here, we demonstrate that schizophrenia involves an aberrant topology of the structural infrastructure of the brain network.	topic_sch
75846	1	355327	7	NULL	NULL	0	NULL	Senescence	Process		implicated as					tumor suppression	Process	mechanism of			NULL		0	NULL	NULL	NULL	NULL	NULL	Senescence has been implicated as an important mechanism of tumour suppression in a number of human malignancies, including colorectal cancer (CRC).	topic_ccc
75847	2	355327	7	NULL	NULL	0	NULL	statement 1	Process		occur in					CRC	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Senescence has been implicated as an important mechanism of tumour suppression in a number of human malignancies, including colorectal cancer (CRC).	topic_ccc
75848	3	355327	7	NULL	NULL	0	NULL	CRC	MedicalFinding		is a type of					human malignancy	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Senescence has been implicated as an important mechanism of tumour suppression in a number of human malignancies, including colorectal cancer (CRC).	topic_ccc
75849	1	355328	7	NULL	NULL	0	NULL	Apc	GP	loss of	induce					senescence	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	n this study we have examined the capacity of Apc loss to induce senescence in the intestinal epithelium compared to the renal epithelium. 	topic_ccc
75850	2	355328	7	NULL	NULL	0	NULL	statement 1	Process		occur in					intestinal epithelium	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	n this study we have examined the capacity of Apc loss to induce senescence in the intestinal epithelium compared to the renal epithelium. 	topic_ccc
75862	1	355330	7	NULL	NULL	0	NULL	 Apc function	Process	loss of	leads to					senescence	Process	induction of			NULL		0	NULL	NULL	NULL	NULL	NULL	Within the renal epithelium, loss of Apc function led to an induction of senescence, however, bypassing senescence through combined Apc and p21 or Ink4A gene deletion rapidly initiated renal carcinoma. 	topic_ccc
75863	2	355330	7	NULL	NULL	0	NULL	statement 1	Process		occur in					renal epithelium	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Within the renal epithelium, loss of Apc function led to an induction of senescence, however, bypassing senescence through combined Apc and p21 or Ink4A gene deletion rapidly initiated renal carcinoma. 	topic_ccc
75864	3	355330	7	NULL	NULL	0	NULL	Apc	GP		combined with					p21	GP	gene deletion of			NULL		0	NULL	NULL	NULL	NULL	NULL	Within the renal epithelium, loss of Apc function led to an induction of senescence, however, bypassing senescence through combined Apc and p21 or Ink4A gene deletion rapidly initiated renal carcinoma. 	topic_ccc
75865	4	355330	7	NULL	NULL	0	NULL	Apc	GP		combined with					Ink4A	GP	gene deletion of			NULL		0	NULL	NULL	NULL	NULL	NULL	Within the renal epithelium, loss of Apc function led to an induction of senescence, however, bypassing senescence through combined Apc and p21 or Ink4A gene deletion rapidly initiated renal carcinoma. 	topic_ccc
75866	5	355330	7	NULL	NULL	0	NULL	statement 3	Process		initiate		rapidly			renal carcinoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Within the renal epithelium, loss of Apc function led to an induction of senescence, however, bypassing senescence through combined Apc and p21 or Ink4A gene deletion rapidly initiated renal carcinoma. 	topic_ccc
75867	6	355330	7	NULL	NULL	0	NULL	statement 4	Process		initiate		rapidly			renal carcinoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Within the renal epithelium, loss of Apc function led to an induction of senescence, however, bypassing senescence through combined Apc and p21 or Ink4A gene deletion rapidly initiated renal carcinoma. 	topic_ccc
75868	7	355330	7	NULL	NULL	0	NULL	senescence 	Process	bypassing	leads to					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Within the renal epithelium, loss of Apc function led to an induction of senescence, however, bypassing senescence through combined Apc and p21 or Ink4A gene deletion rapidly initiated renal carcinoma. 	topic_ccc
75869	8	355330	7	NULL	NULL	0	NULL	senescence 	Process	bypassing	leads to					statement 6	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Within the renal epithelium, loss of Apc function led to an induction of senescence, however, bypassing senescence through combined Apc and p21 or Ink4A gene deletion rapidly initiated renal carcinoma. 	topic_ccc
75870	1	355331	7	NULL	NULL	0	NULL	cancer stem cells	Cell		limitation for 		severe			cancer	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	cancer stem or tumor-initiating cells (TICs) are a severe limitation for the treatment of cancer by conventional therapies.	topic_ccc
75871	2	355331	7	NULL	NULL	NULL	NULL	TICs	Cell		limitation for 		severe			cancer	MedicalFinding	treatment of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	cancer stem or tumor-initiating cells (TICs) are a severe limitation for the treatment of cancer by conventional therapies.	topic_ccc
75872	3	355331	7	NULL	NULL	0	NULL	TICs	Cell		is					tumor-initiating cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	cancer stem or tumor-initiating cells (TICs) are a severe limitation for the treatment of cancer by conventional therapies.	topic_ccc
75873	1	355332	7	NULL	NULL	0	NULL	MT110	Chemical		recognizes					EpCAM	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	MT110 recognizes EpCAM, a cell adhesion molecule expressed on TICs from diverse human carcinoma	topic_ccc
75874	2	355332	7	NULL	NULL	0	NULL	EpCAM	GP		is a type of					cell adhesion molecule	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	MT110 recognizes EpCAM, a cell adhesion molecule expressed on TICs from diverse human carcinoma	topic_ccc
75875	3	355332	7	NULL	NULL	0	NULL	EpCAM	GP		expressed on					TICs	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	MT110 recognizes EpCAM, a cell adhesion molecule expressed on TICs from diverse human carcinoma	topic_ccc
75876	4	355332	7	NULL	NULL	0	NULL	statement 3	Process		occur in					diverse human carcinoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	MT110 recognizes EpCAM, a cell adhesion molecule expressed on TICs from diverse human carcinoma	topic_ccc
75877	1	355334	7	NULL	NULL	0	NULL	MT110	Chemical		mediates		highly;;potent			 KRAS	GP	complete redirected lysis of			NULL		0	NULL	NULL	NULL	NULL	NULL	 MT110 was highly potent in mediating complete redirected lysis of KRAS-, PI3 kinase- and BRAF-mutated colorectal TICs, as demonstrated in a soft agar assay	topic_ccc
75878	2	355334	7	NULL	NULL	0	NULL	MT110	Chemical		mediates		highly;;potent			PI3 kinase	GP	complete redirected lysis of			NULL		0	NULL	NULL	NULL	NULL	NULL	 MT110 was highly potent in mediating complete redirected lysis of KRAS-, PI3 kinase- and BRAF-mutated colorectal TICs, as demonstrated in a soft agar assay	topic_ccc
75879	3	355334	7	NULL	NULL	NULL	NULL	MT110	Chemical		mediates		highly;;potent			colorectal TICs	Cell	complete redirected lysis of;;BRAF-mutated 			NULL		NULL	NULL	NULL	NULL	NULL	NULL	 MT110 was highly potent in mediating complete redirected lysis of KRAS-, PI3 kinase- and BRAF-mutated colorectal TICs, as demonstrated in a soft agar assay	topic_ccc
75880	1	355335	7	NULL	NULL	NULL	NULL	neoadjuvant chemoradiotherapy 	MedicalProcedure		improve					rectal carcinoma	MedicalFinding	local recurrence rates of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	There is substantial evidence for neoadjuvant chemoradiotherapy and extended abdominoperineal excision (APE) for improving local recurrence rates and overall survival for rectal carcinoma	topic_ccc
75881	2	355335	7	NULL	NULL	0	NULL	APE	MedicalProcedure		improve					rectal carcinoma	MedicalFinding	local recurrence rates of			NULL		0	NULL	NULL	NULL	NULL	NULL	There is substantial evidence for neoadjuvant chemoradiotherapy and extended abdominoperineal excision (APE) for improving local recurrence rates and overall survival for rectal carcinoma	topic_ccc
75882	3	355335	7	NULL	NULL	0	NULL	neoadjuvant chemoradiotherapy	MedicalProcedure		improve					rectal carcinoma	MedicalFinding	overall survival for			NULL		0	NULL	NULL	NULL	NULL	NULL	There is substantial evidence for neoadjuvant chemoradiotherapy and extended abdominoperineal excision (APE) for improving local recurrence rates and overall survival for rectal carcinoma	topic_ccc
75883	4	355335	7	NULL	NULL	0	NULL	APE	MedicalProcedure		improve					rectal carcinoma	MedicalFinding	overall survival for			NULL		0	NULL	NULL	NULL	NULL	NULL	There is substantial evidence for neoadjuvant chemoradiotherapy and extended abdominoperineal excision (APE) for improving local recurrence rates and overall survival for rectal carcinoma	topic_ccc
75884	5	355335	7	NULL	NULL	0	NULL	APE	MedicalProcedure		is					abdominoperineal excision	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	There is substantial evidence for neoadjuvant chemoradiotherapy and extended abdominoperineal excision (APE) for improving local recurrence rates and overall survival for rectal carcinoma	topic_ccc
75885	1	355336	7	NULL	NULL	NULL	NULL	bipolar disorder	MedicalFinding		have					small amygdalae	OrganismPart				NULL		NULL	NULL	NULL	NULL	NULL	NULL	There are a number of studies that show that children with bipolar disorder have small amygdalae compared to controls. There’s also evidence that their amygdalae, although small, may also be overactive. NULL	topic_bd
75886	2	355336	7	NULL	NULL	NULL	NULL	small amygdalae	OrganismPart		may be					overactive	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	There are a number of studies that show that children with bipolar disorder have small amygdalae compared to controls. There’s also evidence that their amygdalae, although small, may also be overactive. NULL	topic_bd
75887	1	355338	7	NULL	NULL	0	NULL	right amygdala	OrganismPart		located inside					brain	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	There’s a right and left amygdala, and they’re located deep inside the brain roughly on a line from your temples. They are one of the parts of the brain that govern emotions.	topic_bd
75888	2	355338	7	NULL	NULL	0	NULL	left amygdala	OrganismPart		located inside					brain	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	There’s a right and left amygdala, and they’re located deep inside the brain roughly on a line from your temples. They are one of the parts of the brain that govern emotions.	topic_bd
75889	3	355338	7	NULL	NULL	0	NULL	statement 1	Process		govern					emotions	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	There’s a right and left amygdala, and they’re located deep inside the brain roughly on a line from your temples. They are one of the parts of the brain that govern emotions.	topic_bd
75890	4	355338	7	NULL	NULL	0	NULL	statement 2	Process		govern					emotions	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	There’s a right and left amygdala, and they’re located deep inside the brain roughly on a line from your temples. They are one of the parts of the brain that govern emotions.	topic_bd
75891	1	355339	7	NULL	NULL	0	NULL	dangerous things	MentalProcess		capture					amygdalae	OrganismPart	attention of			NULL		0	NULL	NULL	NULL	NULL	NULL	Things that are really dangerous or really rewarding capture the attention of the amygdalae. 	topic_bd
75892	2	355339	7	NULL	NULL	0	NULL	rewarding things	MentalProcess		capture					amygdalae	OrganismPart	attention of			NULL		0	NULL	NULL	NULL	NULL	NULL	Things that are really dangerous or really rewarding capture the attention of the amygdalae. 	topic_bd
75893	1	355340	7	NULL	NULL	0	NULL	ADHD	MedicalFinding	children with	similar to					bipolar disorder	MedicalFinding	children with			NULL		0	NULL	NULL	NULL	NULL	NULL	What we’re finding is that these very irritable children with ADHD share some characteristics with children with bipolar disorder, but also have significant differences.	topic_bd
75894	2	355340	7	NULL	NULL	NULL	NULL	ADHD	MedicalFinding	children with	differ in		significantly			bipolar disorder	MedicalFinding	children with			NULL		NULL	NULL	NULL	NULL	NULL	NULL	What we’re finding is that these very irritable children with ADHD share some characteristics with children with bipolar disorder, but also have significant differences.	topic_bd
75895	1	355342	7	NULL	NULL	0	NULL	Classic bipolar disorder	MedicalFinding		characterized by					episodes	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Classic bipolar disorder is characterized by episodes.	topic_bd
75896	1	355343	7	NULL	NULL	0	NULL	bipolar	MedicalFinding		severely					mood dysregulated	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	One term being applied to these children who don’t quite fit the definition of bipolar is severely mood dysregulated, or S.M.D.	topic_bd
75897	2	355343	7	NULL	NULL	0	NULL	SMD	MedicalFinding		is					severely mood dysregulated	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	One term being applied to these children who don’t quite fit the definition of bipolar is severely mood dysregulated, or S.M.D.	topic_bd
75898	1	355344	7	NULL	NULL	0	NULL	prefrontal cortex	OrganismPart		damp down					amygdalae	OrganismPart	activity of			NULL		0	NULL	NULL	NULL	NULL	NULL	For example, we know that one action of the prefrontal cortex is to damp down the activity of the amygdalae. So in terms of treatment of bipolar disorder, where the amygdalae may be overactive, we’re thinking about whether we might be able to teach or stimulate the prefrontal cortex to damp down the amygdalae more. 	topic_bd
75899	1	355345	7	NULL	NULL	NULL	NULL	family-focused therapy	MedicalProcedure		help in					patient illness	MedicalFinding	managing			NULL		NULL	NULL	NULL	NULL	NULL	NULL	family-focused therapy the point is not to treat relatives, but to enlist their help in managing the patient’s illness.	topic_bd
75900	1	355346	7	NULL	NULL	0	NULL	 family-focused therapy	MedicalFinding		help in					episodes	MedicalFinding	quicker recoveries from			NULL		0	NULL	NULL	NULL	NULL	NULL	consistently find that if you combine medication and family-focused therapy, you get quicker recoveries from episodes and longer intervals of wellness	topic_bd
75901	2	355346	7	NULL	NULL	0	NULL	medication	MedicalProcedure		help in					episodes	MedicalFinding	quicker recoveries from			NULL		0	NULL	NULL	NULL	NULL	NULL	consistently find that if you combine medication and family-focused therapy, you get quicker recoveries from episodes and longer intervals of wellness	topic_bd
75902	1	355347	7	NULL	NULL	0	NULL	Cep55/c10orf3 	GP	expression of	collated with					CRC	MedicalFinding	high histological grade of 			NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty-three percent cases showed weak positive for Cep55/c10orf3 in total 70 CRC cases. The Cep55/c10orf3 expression intention was collated with high histological grade of CRC.	topic_ccc
75903	1	355348	7	NULL	NULL	0	NULL	Cep55/c10orf3 	GP	peptide from	targeted by					CTLs					NULL	PBMCs	0	NULL	NULL	NULL	NULL	NULL	In our previous study, we demonstrated that a peptide derived from the novel centrosome residing protein Cep55/c10orf3 can be targeted by the cytotoxic T lymphocytes (CTLs) in peripheral blood mononuclear cells (PBMCs) of breast carcinoma patients.	topic_ccc
75904	2	355348	7	NULL	NULL	0	NULL	statement 1	Process		occur in					breast carcinoma patients	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In our previous study, we demonstrated that a peptide derived from the novel centrosome residing protein Cep55/c10orf3 can be targeted by the cytotoxic T lymphocytes (CTLs) in peripheral blood mononuclear cells (PBMCs) of breast carcinoma patients.	topic_ccc
75905	3	355348	7	NULL	NULL	0	NULL	CTLs	Cell		is					cytotoxic T lymphocytes	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	In our previous study, we demonstrated that a peptide derived from the novel centrosome residing protein Cep55/c10orf3 can be targeted by the cytotoxic T lymphocytes (CTLs) in peripheral blood mononuclear cells (PBMCs) of breast carcinoma patients.	topic_ccc
75906	4	355348	7	NULL	NULL	0	NULL	PBMCs	Cell		is					peripheral blood mononuclear cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	In our previous study, we demonstrated that a peptide derived from the novel centrosome residing protein Cep55/c10orf3 can be targeted by the cytotoxic T lymphocytes (CTLs) in peripheral blood mononuclear cells (PBMCs) of breast carcinoma patients.	topic_ccc
75907	5	355348	7	NULL	NULL	0	NULL	Cep55/c10orf3	GP		is a type of					novel centrosome residing protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	In our previous study, we demonstrated that a peptide derived from the novel centrosome residing protein Cep55/c10orf3 can be targeted by the cytotoxic T lymphocytes (CTLs) in peripheral blood mononuclear cells (PBMCs) of breast carcinoma patients.	topic_ccc
75908	1	355349	7	NULL	NULL	NULL	NULL	Methylation	Process	 tolerance of	occur due to					MGMT	GP	field defect in			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Methylation tolerance due to an O6-methylguanine DNA methyltransferase (MGMT) field defect in the colonic mucosa: an initiating step in the development of mismatch repair-deficient colorectal cancers.	topic_ccc
75909	2	355349	7	NULL	NULL	0	NULL	statement 1	Process		occur in					colonic mucosa	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Methylation tolerance due to an O6-methylguanine DNA methyltransferase (MGMT) field defect in the colonic mucosa: an initiating step in the development of mismatch repair-deficient colorectal cancers.	topic_ccc
75910	3	355349	7	NULL	NULL	NULL	NULL	MGMT	GP		is					O6-methylguanine DNA methyltransferase	GP				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Methylation tolerance due to an O6-methylguanine DNA methyltransferase (MGMT) field defect in the colonic mucosa: an initiating step in the development of mismatch repair-deficient colorectal cancers.	topic_ccc
75911	4	355349	7	NULL	NULL	0	NULL	Methylation	Process	tolerance in	initiating step in					mismatch repair-deficient colorectal cancers	MedicalFinding	development of			NULL		0	NULL	NULL	NULL	NULL	NULL	Methylation tolerance due to an O6-methylguanine DNA methyltransferase (MGMT) field defect in the colonic mucosa: an initiating step in the development of mismatch repair-deficient colorectal cancers.	topic_ccc
75912	1	355350	7	NULL	NULL	0	NULL	HSP27	GP		prognostic indicator in					rectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Low molecular weight heat shock protein HSP27 is a prognostic indicator in rectal cancer but not colon cancer.	topic_ccc
75913	2	355350	7	NULL	NULL	0	NULL	HSP27	GP		is not a prognostic indicator in					colon cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Low molecular weight heat shock protein HSP27 is a prognostic indicator in rectal cancer but not colon cancer.	topic_ccc
75914	3	355350	7	NULL	NULL	0	NULL	HSP27	GP		is a type of					Low molecular weight heat shock protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Low molecular weight heat shock protein HSP27 is a prognostic indicator in rectal cancer but not colon cancer.	topic_ccc
75915	1	355351	7	NULL	NULL	NULL	NULL	P-LVD	OrganismPart	high density of	associated with					VEGF	GP	high expression of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	 Results A high density of peritumoural lymphatics (P-LVD) was significantly associated with high VEGF expression and disease progression.	topic_ccc
75916	2	355351	7	NULL	NULL	NULL	NULL	P-LVD	OrganismPart	high density of	associated with					disease progression	Process	high			NULL		NULL	NULL	NULL	NULL	NULL	NULL	 Results A high density of peritumoural lymphatics (P-LVD) was significantly associated with high VEGF expression and disease progression.	topic_ccc
75917	3	355351	7	NULL	NULL	0	NULL	P-LVD	OrganismPart		is					 peritumoural lymphatics	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	 Results A high density of peritumoural lymphatics (P-LVD) was significantly associated with high VEGF expression and disease progression.	topic_ccc
74411	1	355353	5	NULL	NULL	0	NULL	VENTX	GP		is					Vent-like homeobox gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Vent-like homeobox gene VENTX, a putative homolog of the Xenopus xvent2 gene, 	topic_ll
74412	2	355353	5	NULL	NULL	0	NULL	VENTX	GP		is a homolog of		putative			xvent2 gene	GP	Xenopus			NULL		0	NULL	NULL	NULL	NULL	NULL	Vent-like homeobox gene VENTX, a putative homolog of the Xenopus xvent2 gene, 	topic_ll
74413	1	355354	5	NULL	NULL	0	NULL	VENTX	GP		is					Vent-like homeobox gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The vent-like homeobox gene VENTX promotes human myeloid differentiation 	topic_ll
74414	2	355354	5	NULL	NULL	0	NULL	VENTX	GP		promotes					myeloid differentiation	Process	human			NULL		0	NULL	NULL	NULL	NULL	NULL	The vent-like homeobox gene VENTX promotes human myeloid differentiation 	topic_ll
74415	1	355356	5	NULL	NULL	0	NULL	RIZ1 gene	GP		is inactivated in		partly			MDS	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	RIZ1 gene is inactivated in MDS and AML in part by methylation, 	topic_ll
74416	2	355356	5	NULL	NULL	0	NULL	RIZ1 gene	GP		is inactivated in		partly			AML	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	RIZ1 gene is inactivated in MDS and AML in part by methylation, 	topic_ll
74417	3	355356	5	NULL	NULL	0	NULL	methylation	Process		plays a role in					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	RIZ1 gene is inactivated in MDS and AML in part by methylation, 	topic_ll
74418	4	355356	5	NULL	NULL	0	NULL	methylation	Process		plays a role in					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	RIZ1 gene is inactivated in MDS and AML in part by methylation, 	topic_ll
74419	1	355359	5	NULL	NULL	0	NULL	FOXM1	GP	aberrant expression of	induce					AML cell	Cell	 proliferation of			NULL		0	NULL	NULL	NULL	NULL	NULL	aberrant expression of FOXM1 induces AML cell proliferation through modulation of cell cycle progression.	topic_ll
74420	2	355359	5	NULL	NULL	0	NULL	statement 1	Process		occurs through					cell cycle progression	Process	modulation of			NULL		0	NULL	NULL	NULL	NULL	NULL	aberrant expression of FOXM1 induces AML cell proliferation through modulation of cell cycle progression.	topic_ll
74421	1	355361	5	NULL	NULL	0	NULL	amplicons	Chromosome		is expressed in					breast cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Retinoic acid receptor alpha (RARA) and other target sequences at 17p11.2 often represent the amplicons expressed in breast cancer, not in AML	topic_ll
74422	2	355361	5	NULL	NULL	0	NULL	RARA	GP		is					retinoic acid receptor alpha	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Retinoic acid receptor alpha (RARA) and other target sequences at 17p11.2 often represent the amplicons expressed in breast cancer, not in AML	topic_ll
74423	3	355361	5	NULL	NULL	0	NULL	RARA	GP		represent					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Retinoic acid receptor alpha (RARA) and other target sequences at 17p11.2 often represent the amplicons expressed in breast cancer, not in AML	topic_ll
74424	4	355361	5	NULL	NULL	0	NULL	target sequences	NucleicAcid		is present in					17p11.2	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	Retinoic acid receptor alpha (RARA) and other target sequences at 17p11.2 often represent the amplicons expressed in breast cancer, not in AML	topic_ll
74425	5	355361	5	NULL	NULL	0	NULL	statement 4	NucleicAcid		represent					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Retinoic acid receptor alpha (RARA) and other target sequences at 17p11.2 often represent the amplicons expressed in breast cancer, not in AML	topic_ll
74426	6	355361	5	NULL	NULL	0	NULL	amplicons	Chromosome		is not expressed in					AML	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Retinoic acid receptor alpha (RARA) and other target sequences at 17p11.2 often represent the amplicons expressed in breast cancer, not in AML	topic_ll
74427	1	355363	5	NULL	NULL	0	NULL	AML cells	Cell		is differentiated into					dendritic cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	AML cells can be differentiated into dendritic cells (AML-DCs), which have increased immunogenicity and have been proposed as vaccines against leukemia. 	topic_ll
74428	2	355363	5	NULL	NULL	0	NULL	statement 1	Cell		is					AML-DCs	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	AML cells can be differentiated into dendritic cells (AML-DCs), which have increased immunogenicity and have been proposed as vaccines against leukemia. 	topic_ll
74429	3	355363	5	NULL	NULL	0	NULL	AML-DCs	Cell		contains					immunogenicity	AbstractConcept	increased			NULL		0	NULL	NULL	NULL	NULL	NULL	AML cells can be differentiated into dendritic cells (AML-DCs), which have increased immunogenicity and have been proposed as vaccines against leukemia. 	topic_ll
74430	4	355363	5	NULL	NULL	0	NULL	AML-DCs	Cell		is a type of					vaccine	AbstractConcept				NULL		0	NULL	NULL	NULL	NULL	NULL	AML cells can be differentiated into dendritic cells (AML-DCs), which have increased immunogenicity and have been proposed as vaccines against leukemia. 	topic_ll
74431	5	355363	5	NULL	NULL	0	NULL	AML-DCs	Cell		acts against					leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	AML cells can be differentiated into dendritic cells (AML-DCs), which have increased immunogenicity and have been proposed as vaccines against leukemia. 	topic_ll
74432	1	355365	5	NULL	NULL	0	NULL	FLT3	GP		is					 fms-like receptor tyrosine kinase-3	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	ms-like receptor tyrosine kinase-3 (FLT3), which is important for the normal development of hematopoietic stem cells and cells of the immune system, is frequently mutated in patients with acute myeloid leukemia (AML). 	topic_ll
74433	2	355365	5	NULL	NULL	0	NULL	FLT3	GP		is important for					hematopoietic stem cells	Cell	normal development of			NULL		0	NULL	NULL	NULL	NULL	NULL	ms-like receptor tyrosine kinase-3 (FLT3), which is important for the normal development of hematopoietic stem cells and cells of the immune system, is frequently mutated in patients with acute myeloid leukemia (AML). 	topic_ll
74434	3	355365	5	NULL	NULL	0	NULL	FLT3	GP		is important for					immune system	OrganismPart	normal development of;;cells of			NULL		0	NULL	NULL	NULL	NULL	NULL	ms-like receptor tyrosine kinase-3 (FLT3), which is important for the normal development of hematopoietic stem cells and cells of the immune system, is frequently mutated in patients with acute myeloid leukemia (AML). 	topic_ll
74435	4	355365	5	NULL	NULL	NULL	NULL	FLT3	GP		is mutated in		frequently			AML patients	GroupOfPeople				NULL		NULL	NULL	NULL	NULL	NULL	NULL	ms-like receptor tyrosine kinase-3 (FLT3), which is important for the normal development of hematopoietic stem cells and cells of the immune system, is frequently mutated in patients with acute myeloid leukemia (AML). 	topic_ll
74436	5	355365	5	NULL	NULL	0	NULL	AML	MedicalFinding		is					acute myeloid leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	ms-like receptor tyrosine kinase-3 (FLT3), which is important for the normal development of hematopoietic stem cells and cells of the immune system, is frequently mutated in patients with acute myeloid leukemia (AML). 	topic_ll
74477	1	355366	5	NULL	NULL	NULL	NULL	FLT3	GP		is mutated in					AML patients	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	FLT3 inhibitors have shown therapeutic activity in AML patients with FLT3 mutations. Sorafenib and sunitinib were the first FLT3 inhibitors to be studied in the clinic and have the most clinically relevant data.	topic_ll
74481	2	355366	5	NULL	NULL	NULL	NULL	FLT3 inhibitors	Chemical		is therapeutically active in					AML patients	GroupOfPeople				NULL		NULL	NULL	NULL	NULL	NULL	NULL	FLT3 inhibitors have shown therapeutic activity in AML patients with FLT3 mutations. Sorafenib and sunitinib were the first FLT3 inhibitors to be studied in the clinic and have the most clinically relevant data.	topic_ll
74483	3	355366	5	NULL	NULL	0	NULL	sunitinib	Chemical		is an inhibitor of					FLT3	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	FLT3 inhibitors have shown therapeutic activity in AML patients with FLT3 mutations. Sorafenib and sunitinib were the first FLT3 inhibitors to be studied in the clinic and have the most clinically relevant data.	topic_ll
74485	4	355366	5	NULL	NULL	0	NULL	sorafenib	Chemical		is an inhibitor of					FLT3	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	FLT3 inhibitors have shown therapeutic activity in AML patients with FLT3 mutations. Sorafenib and sunitinib were the first FLT3 inhibitors to be studied in the clinic and have the most clinically relevant data.	topic_ll
74488	1	355368	5	NULL	NULL	0	NULL	FLT3 inhibitors	Chemical		is therapeutically active in					AML patients	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	FLT3 inhibitors have shown therapeutic activity in AML patients with FLT3 mutations.	topic_ll
74489	2	355368	5	NULL	NULL	0	NULL	FLT3	GP		is mutated in					AML patients	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	FLT3 inhibitors have shown therapeutic activity in AML patients with FLT3 mutations.	topic_ll
74490	1	355369	5	NULL	NULL	0	NULL	formaldehyde	Chemical		cause		potentially			leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Hematological and toxicological evaluation of formaldehyde as a potential cause of human leukemia.	topic_ll
74491	1	355370	5	NULL	NULL	0	NULL	formaldehyde	Chemical	exposure	is associated with					AML	MedicalFinding	higher risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	formaldehyde exposure is associated with a higher risk of acute myelogenous leukemia (AML)	topic_ll
74492	2	355370	5	NULL	NULL	0	NULL	AML	MedicalFinding		is					acute myelogenous leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	formaldehyde exposure is associated with a higher risk of acute myelogenous leukemia (AML)	topic_ll
74493	1	355373	5	NULL	NULL	0	NULL	transplantation	Process	allogeneic	salvage					chemotherapy	MedicalProcedure	failures of			NULL		0	NULL	NULL	NULL	NULL	NULL	Allogeneic transplantation can act as a salvage for chemotherapy failures	topic_ll
74494	1	355376	5	NULL	NULL	0	NULL	SMT-A07	Chemical		induces					leukemia cells	Cell	apoptosis of			NULL	in vitro	0	NULL	NULL	NULL	NULL	NULL	SMT-A07, a 3-(Indol-2-yl) indazole derivative, induces apoptosis of leukemia cells in vitro.	topic_ll
74495	2	355376	5	NULL	NULL	0	NULL	SMT-A07	Chemical		is a derivative of					3-(Indol-2-yl) indazole	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	SMT-A07, a 3-(Indol-2-yl) indazole derivative, induces apoptosis of leukemia cells in vitro.	topic_ll
74496	1	355377	5	NULL	NULL	NULL	NULL	IL-24	GP		induces					chronic lymphocytic leukemia B cells	Cell	apoptosis of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	IL-24 Induces Apoptosis of Chronic Lymphocytic Leukemia B Cells Engaged into the Cell Cycle through Dephosphorylation of STAT3 and Stabilization of p53 Expression	topic_ll
74497	2	355377	5	NULL	NULL	0	NULL	chronic lymphocytic leukemia B cells\t	Cell		engaged in					cell cycle	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	IL-24 Induces Apoptosis of Chronic Lymphocytic Leukemia B Cells Engaged into the Cell Cycle through Dephosphorylation of STAT3 and Stabilization of p53 Expression	topic_ll
74498	3	355377	5	NULL	NULL	0	NULL	statement 1	Process		occurs through					STAT3	GP	dephosphoylation of			NULL		0	NULL	NULL	NULL	NULL	NULL	IL-24 Induces Apoptosis of Chronic Lymphocytic Leukemia B Cells Engaged into the Cell Cycle through Dephosphorylation of STAT3 and Stabilization of p53 Expression	topic_ll
74499	4	355377	5	NULL	NULL	0	NULL	statement 1	Process		occurs through					p53	GP	stabilization of;;expression of			NULL		0	NULL	NULL	NULL	NULL	NULL	IL-24 Induces Apoptosis of Chronic Lymphocytic Leukemia B Cells Engaged into the Cell Cycle through Dephosphorylation of STAT3 and Stabilization of p53 Expression	topic_ll
74616	1	355378	5	NULL	NULL	0	NULL	curcumin	Chemical		downregulates					egr-1	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Curcumin causes the growth arrest and apoptosis of B cell lymphoma by downregulation of egr-1, c-myc, bcl-XL, NF-kappa B, and p53.	topic_ll
74617	2	355378	5	NULL	NULL	0	NULL	statement 1	Process		cause					growth arrest	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Curcumin causes the growth arrest and apoptosis of B cell lymphoma by downregulation of egr-1, c-myc, bcl-XL, NF-kappa B, and p53.	topic_ll
74618	3	355378	5	NULL	NULL	NULL	NULL	statement 1	Process		cause					B cell lymphoma	Cell	apoptosis of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Curcumin causes the growth arrest and apoptosis of B cell lymphoma by downregulation of egr-1, c-myc, bcl-XL, NF-kappa B, and p53.	topic_ll
74619	4	355378	5	NULL	NULL	0	NULL	curcumin	Chemical		downregulates					c-myc	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Curcumin causes the growth arrest and apoptosis of B cell lymphoma by downregulation of egr-1, c-myc, bcl-XL, NF-kappa B, and p53.	topic_ll
74620	5	355378	5	NULL	NULL	0	NULL	statement 4	Process		cause					growth arrest	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Curcumin causes the growth arrest and apoptosis of B cell lymphoma by downregulation of egr-1, c-myc, bcl-XL, NF-kappa B, and p53.	topic_ll
74621	6	355378	5	NULL	NULL	0	NULL	statement 4	Process		cause					B cell lymphoma	Cell	apoptosis of			NULL		0	NULL	NULL	NULL	NULL	NULL	Curcumin causes the growth arrest and apoptosis of B cell lymphoma by downregulation of egr-1, c-myc, bcl-XL, NF-kappa B, and p53.	topic_ll
74622	7	355378	5	NULL	NULL	0	NULL	curcumin	Chemical		downregulates					bcl-XL	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Curcumin causes the growth arrest and apoptosis of B cell lymphoma by downregulation of egr-1, c-myc, bcl-XL, NF-kappa B, and p53.	topic_ll
74623	8	355378	5	NULL	NULL	0	NULL	statement 7	Process		cause					growth arrest	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Curcumin causes the growth arrest and apoptosis of B cell lymphoma by downregulation of egr-1, c-myc, bcl-XL, NF-kappa B, and p53.	topic_ll
74624	9	355378	5	NULL	NULL	0	NULL	statement 7	Process		cause					B cell lymphoma	Cell	apoptosis of			NULL		0	NULL	NULL	NULL	NULL	NULL	Curcumin causes the growth arrest and apoptosis of B cell lymphoma by downregulation of egr-1, c-myc, bcl-XL, NF-kappa B, and p53.	topic_ll
74625	10	355378	5	NULL	NULL	0	NULL	curcumin	Chemical		downregulates					NF-kappa B	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Curcumin causes the growth arrest and apoptosis of B cell lymphoma by downregulation of egr-1, c-myc, bcl-XL, NF-kappa B, and p53.	topic_ll
74626	11	355378	5	NULL	NULL	0	NULL	statement 10	Process		cause					growth arrest	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Curcumin causes the growth arrest and apoptosis of B cell lymphoma by downregulation of egr-1, c-myc, bcl-XL, NF-kappa B, and p53.	topic_ll
74627	12	355378	5	NULL	NULL	0	NULL	statement 10	Process		cause					B cell lymphoma	Cell	apoptosis of			NULL		0	NULL	NULL	NULL	NULL	NULL	Curcumin causes the growth arrest and apoptosis of B cell lymphoma by downregulation of egr-1, c-myc, bcl-XL, NF-kappa B, and p53.	topic_ll
74628	13	355378	5	NULL	NULL	0	NULL	curcumin	Chemical		downregulates					p53	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Curcumin causes the growth arrest and apoptosis of B cell lymphoma by downregulation of egr-1, c-myc, bcl-XL, NF-kappa B, and p53.	topic_ll
74629	14	355378	5	NULL	NULL	0	NULL	statement 13	Process		cause					growth arrest	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Curcumin causes the growth arrest and apoptosis of B cell lymphoma by downregulation of egr-1, c-myc, bcl-XL, NF-kappa B, and p53.	topic_ll
74630	15	355378	5	NULL	NULL	0	NULL	statement 13	Process		cause					B cell lymphoma	Cell	apoptosis of			NULL		0	NULL	NULL	NULL	NULL	NULL	Curcumin causes the growth arrest and apoptosis of B cell lymphoma by downregulation of egr-1, c-myc, bcl-XL, NF-kappa B, and p53.	topic_ll
77680	1	355385	6	NULL	NULL	0	NULL	EGF receptor	GP		plays a role in					Breast cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	at least two of these receptors, the EGF receptor and HER2, play a role in breast cancer	topic_bc
77681	2	355385	6	NULL	NULL	0	NULL	HER2	GP		plays a role in					Breast cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	at least two of these receptors, the EGF receptor and HER2, play a role in breast cancer	topic_bc
77682	1	355386	6	NULL	NULL	0	NULL	Tenascin-C	Chemical		stimulates					cell proliferation	Process				NULL	cancer	0	NULL	NULL	NULL	NULL	NULL	Tenascin-C stimulates cancer cell proliferation. 	topic_bc
77683	1	355387	6	NULL	NULL	0	NULL	Breast cancer	MedicalFinding		causes 					TNC	GP	upregulation of			NULL		0	NULL	NULL	NULL	NULL	NULL	The ECM protein tenascin-C (TNC) is frequently up-regulated in breast cancer	topic_bc
77684	2	355387	6	NULL	NULL	0	NULL	Tenascin-C	GP		is a type of					ECM protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The ECM protein tenascin-C (TNC) is frequently up-regulated in breast cancer	topic_bc
77685	3	355387	6	NULL	NULL	0	NULL	TNC	GP		is					tenascin-C	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The ECM protein tenascin-C (TNC) is frequently up-regulated in breast cancer	topic_bc
77686	1	355388	6	NULL	NULL	NULL	NULL	Estradiol	GP		plays a role in		critical			breast cancer 	MedicalFinding	sporadic;; progression of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Estradiol (E2) play a critical role in sporadic breast cancer progression and decrease apoptosis in breast cancer cells	topic_bc
77687	2	355388	6	NULL	NULL	0	NULL	Estradiol	GP		decrease					apoptosis	Process				NULL	breast cancer cells	0	NULL	NULL	NULL	NULL	NULL	Estradiol (E2) play a critical role in sporadic breast cancer progression and decrease apoptosis in breast cancer cells	topic_bc
77735	3	355388	6	NULL	NULL	0	NULL	Estradiol	GP		is					E2	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Estradiol (E2) play a critical role in sporadic breast cancer progression and decrease apoptosis in breast cancer cells	topic_bc
77736	1	355389	6	NULL	NULL	0	NULL	tamoxifen	Chemical		acts as					Breast cancer 	MedicalFinding	drug for			NULL		0	NULL	NULL	NULL	NULL	NULL	The widely used breast cancer drug tamoxifen (Nolvadex®), which can become less effective over time, might retain its full strength indefinitely if used along with a second drug	topic_bc
77737	2	355389	6	NULL	NULL	0	NULL	tamoxifen	Chemical		is					Nolvadex	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The widely used breast cancer drug tamoxifen (Nolvadex®), which can become less effective over time, might retain its full strength indefinitely if used along with a second drug	topic_bc
77738	1	355390	6	NULL	NULL	0	NULL	tumor	Cell	growth of	is a result of					proliferation	Process	uncontrolled			NULL		0	NULL	NULL	NULL	NULL	NULL	 tumour growth is not just a result of uncontrolled proliferation but also of reduced apoptosis.	topic_bc
77739	2	355390	6	NULL	NULL	0	NULL	tumor	Cell	growth of	is a result of					apoptosis	Process	reduction of 			NULL		0	NULL	NULL	NULL	NULL	NULL	 tumour growth is not just a result of uncontrolled proliferation but also of reduced apoptosis.	topic_bc
77740	1	355391	6	NULL	NULL	0	NULL	Nitric oxide	Chemical		increases					glucose	Chemical	transport of			NULL	breast cancer cells	0	NULL	NULL	NULL	NULL	NULL	Nitric oxide will increase glucose transport in breast cancer cells more than in normal breast cells	topic_bc
77741	2	355391	6	NULL	NULL	0	NULL	Nitric oxide	Chemical		increases					glucose	Chemical	transport of			NULL	normal breast cells	0	NULL	NULL	NULL	NULL	NULL	Nitric oxide will increase glucose transport in breast cancer cells more than in normal breast cells	topic_bc
77742	3	355391	6	NULL	NULL	NULL	NULL	statement 1	Process		is more as compared to					statement 2	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nitric oxide will increase glucose transport in breast cancer cells more than in normal breast cells	topic_bc
77743	2	355392	6	NULL	NULL	NULL	NULL	Breast cancer cell	Cell		uses 					statement 1	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ability of a cancer cell to grow ultimately depends on its ability to take up and metabolize fuel. The primary fuel that is used by the breast cancer cell is carbohydrate. Nitric oxide may regulate the uptake of carbohydrate ultimately affecting its ability to cause hypertrophy in tissues such as skeletal muscle. 	topic_bc
77744	1	355392	6	NULL	NULL	0	NULL	Carbohydrate	Chemical		is used as					primary fuel					NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of a cancer cell to grow ultimately depends on its ability to take up and metabolize fuel. The primary fuel that is used by the breast cancer cell is carbohydrate. Nitric oxide may regulate the uptake of carbohydrate ultimately affecting its ability to cause hypertrophy in tissues such as skeletal muscle. 	topic_bc
77745	3	355392	6	NULL	NULL	0	NULL	Nitric oxide	Chemical		regulate		may			carbohydrate	Chemical	uptake of 			NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of a cancer cell to grow ultimately depends on its ability to take up and metabolize fuel. The primary fuel that is used by the breast cancer cell is carbohydrate. Nitric oxide may regulate the uptake of carbohydrate ultimately affecting its ability to cause hypertrophy in tissues such as skeletal muscle. 	topic_bc
77746	4	355392	6	NULL	NULL	0	NULL	hypertrophy	MedicalFinding		is caused in 					skeletal muscle	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of a cancer cell to grow ultimately depends on its ability to take up and metabolize fuel. The primary fuel that is used by the breast cancer cell is carbohydrate. Nitric oxide may regulate the uptake of carbohydrate ultimately affecting its ability to cause hypertrophy in tissues such as skeletal muscle. 	topic_bc
77747	5	355392	6	NULL	NULL	0	NULL	statement 3	Process		affects					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of a cancer cell to grow ultimately depends on its ability to take up and metabolize fuel. The primary fuel that is used by the breast cancer cell is carbohydrate. Nitric oxide may regulate the uptake of carbohydrate ultimately affecting its ability to cause hypertrophy in tissues such as skeletal muscle. 	topic_bc
77748	1	355394	6	NULL	NULL	0	NULL	estrogen	GP		increases					Breast cancer	MedicalFinding	occurrence of 			NULL		0	NULL	NULL	NULL	NULL	NULL	Some kinds of breast cancer are fueled by high amounts of estrogen. That's the reason that estrogen suppression medications are an important part of treatment that prevents recurrence	topic_bc
77749	1	355395	6	NULL	NULL	0	NULL	Breast cancer	MedicalFinding		spreads beyond the					breast	cell				NULL		0	NULL	NULL	NULL	NULL	NULL	When breast cancer spreads beyond the breast, it is said to be metastatic	topic_bc
77750	2	355395	6	NULL	NULL	0	NULL	statement 1	Process		is 					metastatic	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	When breast cancer spreads beyond the breast, it is said to be metastatic	topic_bc
77751	1	355396	6	NULL	NULL	0	NULL	estrogen	Chemical	higher levels of	leads to					Breast cancer	MedicalFinding	reoccurence of 			NULL		0	NULL	NULL	NULL	NULL	NULL	It appears that the higher a breast cancer survivor's level of estrogen is the greater is her risk of developing breast cancer again	topic_bc
77752	1	355397	6	NULL	NULL	0	NULL	DLC-1	GP		acts as 					metastasis-suppressor gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The finding that DLC-1 can act as a metastasis-suppressor gene	topic_bc
77753	1	355401	6	NULL	NULL	NULL	NULL	Capecitabine	Chemical		is used in					breast cancer	MedicalFinding	metastatic;; treatment of 			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Capecitabine (INN Xeloda, Roche) is an orally-administered chemotherapeutic agent used in the treatment of metastatic breast and colorectal cancers	topic_bc
77754	2	355401	6	NULL	NULL	0	NULL	Capecitabine	Chemical		is used in					colorectal cancer	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	Capecitabine (INN Xeloda, Roche) is an orally-administered chemotherapeutic agent used in the treatment of metastatic breast and colorectal cancers	topic_bc
74634	1	355404	5	NULL	NULL	0	NULL	JMML	MedicalFinding		is					Juvenile Myelomonocytic Leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Juvenile Myelomonocytic Leukemia (JMML) is a rare form of leukemia which affects young children, generally under the age of five.	topic_ll
74635	2	355404	5	NULL	NULL	0	NULL	JMML	MedicalFinding		is a form of		rare			leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Juvenile Myelomonocytic Leukemia (JMML) is a rare form of leukemia which affects young children, generally under the age of five.	topic_ll
74636	3	355404	5	NULL	NULL	0	NULL	JMML	MedicalFinding		affect					children	GroupOfPeople	young			NULL		0	NULL	NULL	NULL	NULL	NULL	Juvenile Myelomonocytic Leukemia (JMML) is a rare form of leukemia which affects young children, generally under the age of five.	topic_ll
74637	1	355405	5	NULL	NULL	0	NULL	CLL	MedicalFinding		is					Chronic lymphocytic leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic lymphocytic leukemia (CLL) is one of four main types of leukemia. 	topic_ll
74638	2	355405	5	NULL	NULL	0	NULL	CLL	MedicalFinding		is a type of					leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic lymphocytic leukemia (CLL) is one of four main types of leukemia. 	topic_ll
74639	1	355406	5	NULL	NULL	0	NULL	CLL	MedicalFinding		is					Chronic lymphocytic leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic lymphocytic leukemia (chronic lymphoid leukemia, CLL) is a monoclonal disorder	topic_ll
74640	2	355406	5	NULL	NULL	0	NULL	CLL	MedicalFinding		is					chronic lymphoid leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic lymphocytic leukemia (chronic lymphoid leukemia, CLL) is a monoclonal disorder	topic_ll
74641	3	355406	5	NULL	NULL	0	NULL	CLL	MedicalFinding		is a type of					monoclonal disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic lymphocytic leukemia (chronic lymphoid leukemia, CLL) is a monoclonal disorder	topic_ll
77755	1	355407	6	NULL	NULL	0	NULL	Breast carcinoma	MedicalFinding	human	co-express					EGF receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Human breast carcinomas frequently co-express the epidermal growth factor (EGF) receptor and the other three members of the EGF receptor family (HER2, -3 and -4).	topic_bc
77756	2	355407	6	NULL	NULL	0	NULL	Breast carcinoma	MedicalFinding	human	co-express					HER2	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Human breast carcinomas frequently co-express the epidermal growth factor (EGF) receptor and the other three members of the EGF receptor family (HER2, -3 and -4).	topic_bc
77757	3	355407	6	NULL	NULL	0	NULL	Breast carcinoma	MedicalFinding	human	co-express					HER3	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Human breast carcinomas frequently co-express the epidermal growth factor (EGF) receptor and the other three members of the EGF receptor family (HER2, -3 and -4).	topic_bc
77758	4	355407	6	NULL	NULL	0	NULL	Breast carcinoma	MedicalFinding	human	co-express					HER4	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Human breast carcinomas frequently co-express the epidermal growth factor (EGF) receptor and the other three members of the EGF receptor family (HER2, -3 and -4).	topic_bc
77759	5	355407	6	NULL	NULL	0	NULL	HER2	GP		is a type of					EGF receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Human breast carcinomas frequently co-express the epidermal growth factor (EGF) receptor and the other three members of the EGF receptor family (HER2, -3 and -4).	topic_bc
77760	6	355407	6	NULL	NULL	0	NULL	HER3	GP		is a type of					EGF receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Human breast carcinomas frequently co-express the epidermal growth factor (EGF) receptor and the other three members of the EGF receptor family (HER2, -3 and -4).	topic_bc
77761	7	355407	6	NULL	NULL	0	NULL	HER4	GP		is a type of					EGF receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Human breast carcinomas frequently co-express the epidermal growth factor (EGF) receptor and the other three members of the EGF receptor family (HER2, -3 and -4).	topic_bc
78028	1	355410	6	NULL	NULL	0	NULL	fat	Chemical	intake of	is associated with					Breast cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	a positive association between high dietary fat intake and breast cancer	topic_bc
78029	1	355412	6	NULL	NULL	0	NULL	progesterone	Chemical		decreases					Breast cancer	MedicalFinding	risk of 			NULL		0	NULL	NULL	NULL	NULL	NULL	progesterone may actually decrease a woman's risk of breast cancer	topic_bc
78030	1	355413	6	NULL	NULL	0	NULL	early pregnancy	PhysicalPhenomenon		prevents		may			Breast cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	early pregnancy, prolonged lactation, chemical or surgical sterilization, exercise, abstinence from alcohol, and a low-fat diet may help prevent breast cancer	topic_bc
78031	2	355413	6	NULL	NULL	0	NULL	lactation	PhysicalPhenomenon	prolonged	prevents					Breast cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	early pregnancy, prolonged lactation, chemical or surgical sterilization, exercise, abstinence from alcohol, and a low-fat diet may help prevent breast cancer	topic_bc
78032	3	355413	6	NULL	NULL	0	NULL	chemical sterilization	MedicalProcedure		prevents					Breast cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	early pregnancy, prolonged lactation, chemical or surgical sterilization, exercise, abstinence from alcohol, and a low-fat diet may help prevent breast cancer	topic_bc
78033	4	355413	6	NULL	NULL	0	NULL	excercise	PhysicalPhenomenon		prevents					Breast cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	early pregnancy, prolonged lactation, chemical or surgical sterilization, exercise, abstinence from alcohol, and a low-fat diet may help prevent breast cancer	topic_bc
78034	5	355413	6	NULL	NULL	0	NULL	alcohol	Chemical	abstinence from	prevents					Breast cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	early pregnancy, prolonged lactation, chemical or surgical sterilization, exercise, abstinence from alcohol, and a low-fat diet may help prevent breast cancer	topic_bc
78035	6	355413	6	NULL	NULL	0	NULL	low-fat diet			prevents					Breast cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	early pregnancy, prolonged lactation, chemical or surgical sterilization, exercise, abstinence from alcohol, and a low-fat diet may help prevent breast cancer	topic_bc
78036	1	355414	6	NULL	NULL	0	NULL	sterilization	MedicalProcedure		reduce		may			Breast cancer	MedicalFinding	risk of 			NULL		0	NULL	NULL	NULL	NULL	NULL	sterilization may reduce the risk of breast cancer	topic_bc
78037	1	355415	6	NULL	NULL	0	NULL	tamoxifen	Chemical		is used for					Breast cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	tamoxifen is currently used widely in patients with early stage, surgically treated breast cancer and has been shown to decrease contralateral breast cancer by 40%	topic_bc
78038	2	355415	6	NULL	NULL	0	NULL	tamoxifen	Chemical		decrease					contralateral cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	tamoxifen is currently used widely in patients with early stage, surgically treated breast cancer and has been shown to decrease contralateral breast cancer by 40%	topic_bc
78039	1	355416	6	NULL	NULL	0	NULL	skin	OrganismPart	dimpling of	occur due to					Cooper ligament	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	skin dimpling can occur due to tethering of Cooper ligaments from the mass underneath	topic_bc
78040	1	355417	6	NULL	NULL	0	NULL	CHEK2	GP		is					 CHK2 checkpoint homolog	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	CHEK2 is the official symbol for the human gene CHK2 checkpoint homolog.	topic_bc
78042	1	355420	6	NULL	NULL	NULL	NULL	parabens	Chemical		have					estrogen	Chemical	properties of;; weak			NULL	breast cancer tumor	NULL	NULL	NULL	NULL	NULL	NULL	One small study has found trace levels of parabens (used as preservatives in antiperspirants and other products), which have weak estrogen-like properties, in a small sample of breast cancer tumors	topic_bc
78043	1	355421	6	NULL	NULL	0	NULL	Breast cancer	MedicalFinding		have					melatonin	Chemical	low levels of			NULL		0	NULL	NULL	NULL	NULL	NULL	 Many women with breast cancer have lower levels of melatonin than those without	topic_bc
75918	1	355423	7	NULL	NULL	0	NULL	Dopamine	Chemical		is a type of					catecholamine neurotransmitter	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Dopamine is a catecholamine neurotransmitter present in a wide variety of animals	topic_bd
75919	2	355423	7	NULL	NULL	0	NULL	statement 1	Process		occur in					animals	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Dopamine is a catecholamine neurotransmitter present in a wide variety of animals	topic_bd
78044	1	355424	6	NULL	NULL	0	NULL	Rb gene	GP		is located on					chromosome 13q14	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	The Rb gene is located on chromosome 13q14, and loss of this region has been implicated in breast cancer progression.  Structural abnormalities including chromo-somal loss and mutation of the Rb gene have been reported in approximately 20-30% of breast cancers	topic_bc
78045	2	355424	6	NULL	NULL	0	NULL	Rb gene	GP	loss of	leads to					Breast cancer	MedicalFinding	progression of			NULL		0	NULL	NULL	NULL	NULL	NULL	The Rb gene is located on chromosome 13q14, and loss of this region has been implicated in breast cancer progression.  Structural abnormalities including chromo-somal loss and mutation of the Rb gene have been reported in approximately 20-30% of breast cancers	topic_bc
78046	3	355424	6	NULL	NULL	0	NULL	Rb gene	GP	mutation of	leads to					Breast cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The Rb gene is located on chromosome 13q14, and loss of this region has been implicated in breast cancer progression.  Structural abnormalities including chromo-somal loss and mutation of the Rb gene have been reported in approximately 20-30% of breast cancers	topic_bc
78047	1	355426	6	NULL	NULL	0	NULL	BRCA3	GP		is linked to					Breast cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	There is evidence for an additional breast cancer suscep- tibility gene (BRCA3) in families at high risk for breast cancer which do not have linkage to either BRCA1 or BRCA2.	topic_bc
78048	2	355426	6	NULL	NULL	0	NULL	BRCA3			is					breast cancer susceptibility gene					NULL		0	NULL	NULL	NULL	NULL	NULL	There is evidence for an additional breast cancer suscep- tibility gene (BRCA3) in families at high risk for breast cancer which do not have linkage to either BRCA1 or BRCA2.	topic_bc
78049	1	355427	6	NULL	NULL	0	NULL	ATM	GP		is located on					chromosome 11q23	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	ATM is located on 11q23 	topic_bc
78050	1	355428	6	NULL	NULL	0	NULL	PTEN	GP		is mapped to					chromosome 10q23	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	PTEN is a protein phosphatase with homology to tensin, which has been mapped to 10q23	topic_bc
78051	2	355428	6	NULL	NULL	0	NULL	PTEN	GP		is homologous to					tensin	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	PTEN is a protein phosphatase with homology to tensin, which has been mapped to 10q23	topic_bc
78052	3	355428	6	NULL	NULL	0	NULL	PTEN	GP		is a type of					protein phosphatase	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	PTEN is a protein phosphatase with homology to tensin, which has been mapped to 10q23	topic_bc
75920	1	355429	7	NULL	NULL	0	NULL	Estrogen	Chemical		is a type of					female hormone	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Estrogen and progesterone are female hormones that regulate the menstrual cycle and likely serve an important role in the regulation of mood.	topic_bd
75921	2	355429	7	NULL	NULL	0	NULL	Estrogen	Chemical		regulate					menstrual cycle	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Estrogen and progesterone are female hormones that regulate the menstrual cycle and likely serve an important role in the regulation of mood.	topic_bd
75922	3	355429	7	NULL	NULL	0	NULL	Estrogen	Chemical		important role in					mood	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Estrogen and progesterone are female hormones that regulate the menstrual cycle and likely serve an important role in the regulation of mood.	topic_bd
75923	4	355429	7	NULL	NULL	0	NULL	progesterone	Chemical		is a type of					female hormone	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Estrogen and progesterone are female hormones that regulate the menstrual cycle and likely serve an important role in the regulation of mood.	topic_bd
75924	5	355429	7	NULL	NULL	0	NULL	progesterone	Chemical		regulate					menstrual cycle	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Estrogen and progesterone are female hormones that regulate the menstrual cycle and likely serve an important role in the regulation of mood.	topic_bd
75925	6	355429	7	NULL	NULL	0	NULL	progesterone	Chemical		important role in					mood	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Estrogen and progesterone are female hormones that regulate the menstrual cycle and likely serve an important role in the regulation of mood.	topic_bd
75926	1	355430	7	NULL	NULL	0	NULL	menstrual cycle	Process	hormonal shifts of	influence					bipolar symptoms	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	the hormonal shifts of the menstrual cycle likely influence bipolar symptoms, but confirmatory research is lacking. NULL	topic_bd
74642	1	355433	5	NULL	NULL	0	NULL	Philadelphia Chromosome	Chromosome		is					Ph chromosome	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	CML patients have what is called the "Philadelphia Chromosome" (Ph chromosome).	topic_ll
74643	2	355433	5	NULL	NULL	0	NULL	Ph chromosome	Chromosome		is present in					CML patients	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	CML patients have what is called the "Philadelphia Chromosome" (Ph chromosome).	topic_ll
74644	1	355434	5	NULL	NULL	0	NULL	Bcr-Abl cancer gene	GP		cause					CML	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The Bcr and Abl genes combine to make the CML-causing gene called the Bcr-Abl cancer gene. 	topic_ll
74647	1	355435	5	NULL	NULL	0	NULL	SLL	MedicalFinding		is					Small lymphocytic lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Small lymphocytic lymphoma (SLL) A disease with identical physical changes in lymph nodes as CLL. 	topic_ll
74649	2	355435	5	NULL	NULL	0	NULL	lymph nodes	OrganismPart		undergo					physical changes	PhysicalPhenomenon	identical			NULL		0	NULL	NULL	NULL	NULL	NULL	Small lymphocytic lymphoma (SLL) A disease with identical physical changes in lymph nodes as CLL. 	topic_ll
74650	3	355435	5	NULL	NULL	NULL	NULL	statement 2	Process		is a symptom of					SLL	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Small lymphocytic lymphoma (SLL) A disease with identical physical changes in lymph nodes as CLL. 	topic_ll
74651	4	355435	5	NULL	NULL	0	NULL	SLL	MedicalFinding		is similar to					CLL	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Small lymphocytic lymphoma (SLL) A disease with identical physical changes in lymph nodes as CLL. 	topic_ll
74652	1	355436	5	NULL	NULL	0	NULL	sprycel	Chemical		is the brand name of					dasatinib	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Sprycel The brand name for dasatinib	topic_ll
74653	1	355437	5	NULL	NULL	0	NULL	Tasigna	Chemical		is the brand name of					nilotinib	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Tasigna The brand name for nilotinib	topic_ll
74654	1	355439	5	NULL	NULL	0	NULL	benzene	Chemical	long-term exposure	cause		may			AML	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The Environmental Protection Agency (EPA) has determined that long-term exposure to benzene may cause acute myelogenous leukemia (AML).	topic_ll
74655	2	355439	5	NULL	NULL	0	NULL	AML	MedicalFinding		is					acute myelogenous leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The Environmental Protection Agency (EPA) has determined that long-term exposure to benzene may cause acute myelogenous leukemia (AML).	topic_ll
74656	3	355439	5	NULL	NULL	0	NULL	EPA	GroupOfPeople		is					Environmental Protection Agency	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	The Environmental Protection Agency (EPA) has determined that long-term exposure to benzene may cause acute myelogenous leukemia (AML).	topic_ll
74657	4	355439	5	NULL	NULL	0	NULL	EPA	GroupOfPeople		determine					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The Environmental Protection Agency (EPA) has determined that long-term exposure to benzene may cause acute myelogenous leukemia (AML).	topic_ll
74658	1	355441	5	NULL	NULL	0	NULL	HTLV	Organism		is					human T-cell lymphocytotropic virus	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	People infected with human T-cell lymphocytotropic virus (HTLV) or human immunodeficiency virus (HIV) also have an increased probability of developing Hodgkin lymphoma.	topic_ll
74659	2	355441	5	NULL	NULL	0	NULL	HIV	Organism		is					human immunodeficiency virus	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	People infected with human T-cell lymphocytotropic virus (HTLV) or human immunodeficiency virus (HIV) also have an increased probability of developing Hodgkin lymphoma.	topic_ll
74660	3	355441	5	NULL	NULL	NULL	NULL	HIV patients	GroupOfPeople		develops		most likely			Hodgkin lymphoma	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	People infected with human T-cell lymphocytotropic virus (HTLV) or human immunodeficiency virus (HIV) also have an increased probability of developing Hodgkin lymphoma.	topic_ll
74661	4	355441	5	NULL	NULL	0	NULL	HTLV patients	GroupOfPeople		develops		most likely			Hodgkin lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	People infected with human T-cell lymphocytotropic virus (HTLV) or human immunodeficiency virus (HIV) also have an increased probability of developing Hodgkin lymphoma.	topic_ll
74662	1	355443	5	NULL	NULL	0	NULL	immune suppression	Process		plays a role in		may			NHL	MedicalFinding	development of			NULL		0	NULL	NULL	NULL	NULL	NULL	The reasons for the development of NHL are not known. Immune suppression plays a role in certain cases.	topic_ll
74663	1	355445	5	NULL	NULL	0	NULL	farming communities	GroupOfPeople		have high incidence of					NHL	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	There is a higher incidence of NHL in farming communities. Studies suggest that specific ingredients in herbicides and pesticides such as organochlorine, organophosphate and phenoxyacid compounds are linked to lymphoma. 	topic_ll
74664	2	355445	5	NULL	NULL	0	NULL	organochlorine	Chemical		plays a role in					lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	There is a higher incidence of NHL in farming communities. Studies suggest that specific ingredients in herbicides and pesticides such as organochlorine, organophosphate and phenoxyacid compounds are linked to lymphoma. 	topic_ll
74665	3	355445	5	NULL	NULL	0	NULL	organophosphate	Chemical		is linked to					lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	There is a higher incidence of NHL in farming communities. Studies suggest that specific ingredients in herbicides and pesticides such as organochlorine, organophosphate and phenoxyacid compounds are linked to lymphoma. 	topic_ll
74666	4	355445	5	NULL	NULL	0	NULL	phenoxyacid compounds	Chemical		is linked to					lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	There is a higher incidence of NHL in farming communities. Studies suggest that specific ingredients in herbicides and pesticides such as organochlorine, organophosphate and phenoxyacid compounds are linked to lymphoma. 	topic_ll
74667	5	355445	5	NULL	NULL	0	NULL	organochlorine	Chemical		is an ingredient of					herbicides	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	There is a higher incidence of NHL in farming communities. Studies suggest that specific ingredients in herbicides and pesticides such as organochlorine, organophosphate and phenoxyacid compounds are linked to lymphoma. 	topic_ll
74668	6	355445	5	NULL	NULL	0	NULL	organochlorine	Chemical		is an ingredient of					pesticides	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	There is a higher incidence of NHL in farming communities. Studies suggest that specific ingredients in herbicides and pesticides such as organochlorine, organophosphate and phenoxyacid compounds are linked to lymphoma. 	topic_ll
74669	7	355445	5	NULL	NULL	0	NULL	organophosphate	Chemical		is an ingredient of					herbicides	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	There is a higher incidence of NHL in farming communities. Studies suggest that specific ingredients in herbicides and pesticides such as organochlorine, organophosphate and phenoxyacid compounds are linked to lymphoma. 	topic_ll
74670	8	355445	5	NULL	NULL	0	NULL	organophosphate	Chemical		is an ingredient of					pesticides	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	There is a higher incidence of NHL in farming communities. Studies suggest that specific ingredients in herbicides and pesticides such as organochlorine, organophosphate and phenoxyacid compounds are linked to lymphoma. 	topic_ll
74671	9	355445	5	NULL	NULL	0	NULL	phenoxyacid compounds	Chemical		is an ingredient of					herbicides	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	There is a higher incidence of NHL in farming communities. Studies suggest that specific ingredients in herbicides and pesticides such as organochlorine, organophosphate and phenoxyacid compounds are linked to lymphoma. 	topic_ll
74672	10	355445	5	NULL	NULL	0	NULL	phenoxyacid compounds	Chemical		is an ingredient of					pesticides	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	There is a higher incidence of NHL in farming communities. Studies suggest that specific ingredients in herbicides and pesticides such as organochlorine, organophosphate and phenoxyacid compounds are linked to lymphoma. 	topic_ll
74673	1	355449	5	NULL	NULL	0	NULL	EBV	Organism		is					Epstein-Barr virus	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Epstein-Barr virus (EBV) infection—in patients from specific geographical regions—is strongly associated with African Burkitt lymphoma.	topic_ll
74674	2	355449	5	NULL	NULL	NULL	NULL	EBV	Organism		infects					specific geographical region	GeographicNotProper	patients of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Epstein-Barr virus (EBV) infection—in patients from specific geographical regions—is strongly associated with African Burkitt lymphoma.	topic_ll
74675	3	355449	5	NULL	NULL	0	NULL	statement 2	Process		is associated with		strongly			African Burkitt lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Epstein-Barr virus (EBV) infection—in patients from specific geographical regions—is strongly associated with African Burkitt lymphoma.	topic_ll
74676	1	355450	5	NULL	NULL	0	NULL	immune systems	OrganismPart		suppressed in					NHL patients	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Epstein-Barr virus infection may play a role in the increased risk of NHL in persons whose immune systems are suppressed as a result of organ transplantation and its associated therapy.	topic_ll
74677	2	355450	5	NULL	NULL	0	NULL	statement 1	Process		is a result of					organ transplantation	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Epstein-Barr virus infection may play a role in the increased risk of NHL in persons whose immune systems are suppressed as a result of organ transplantation and its associated therapy.	topic_ll
74678	3	355450	5	NULL	NULL	0	NULL	Epstein-Barr virus	Organism	infection of	plays a role in					statement 1	Process	increased risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	Epstein-Barr virus infection may play a role in the increased risk of NHL in persons whose immune systems are suppressed as a result of organ transplantation and its associated therapy.	topic_ll
74679	1	355451	5	NULL	NULL	0	NULL	Nodular Sclerosis	MedicalFinding		is a subtype of		most common			Hodgkin lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Nodular Sclerosis is the most common subtype of Hodgkin lymphoma	topic_ll
74680	1	355452	5	NULL	NULL	NULL	NULL	Mixed Cellularity	MedicalFinding		is present in					Hodgkin lymphoma	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mixed Cellularity accounts for about 15 percent to 30 percent of all cases of Hodgkin lymphoma and is found more com­monly in men than women.	topic_ll
74681	2	355452	5	NULL	NULL	0	NULL	statement 1	MedicalFinding		is present in					men	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Mixed Cellularity accounts for about 15 percent to 30 percent of all cases of Hodgkin lymphoma and is found more com­monly in men than women.	topic_ll
74682	3	355452	5	NULL	NULL	0	NULL	statement 1	MedicalFinding		is present in					women	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Mixed Cellularity accounts for about 15 percent to 30 percent of all cases of Hodgkin lymphoma and is found more com­monly in men than women.	topic_ll
74683	4	355452	5	NULL	NULL	0	NULL	statement 2	Process		more common than					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Mixed Cellularity accounts for about 15 percent to 30 percent of all cases of Hodgkin lymphoma and is found more com­monly in men than women.	topic_ll
74684	1	355453	5	NULL	NULL	0	NULL	lymphocyte 	Cell	depletion of	is present in					Hodgkin cases	GroupOfPeople	few			NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocyte Depletion accounts for fewer than 5 percent of all Hodgkin cases.	topic_ll
74685	1	355456	5	NULL	NULL	0	NULL	diffuse lymphocyte predominant	MedicalFinding		is rare than					nodular lymphocyte predominant Hodgkin lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Diffuse Lymphocyte Predominant is extremely rare. The existence of this subtype has been questioned. Most cases are in fact nodular lymphocyte predominant Hodgkin lymphoma with an ill-defined nodular pattern.	topic_ll
74686	1	355457	5	NULL	NULL	0	NULL	monoclonal antibodies	GP		is used to treat		possibly			Hodgkin lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Many promising therapies are currently under investigation in clinical trials for Hodgkin lymphoma. Types of therapy under investigation include: •      Monoclonal antibodies (e.g., SGN-35, which targets the CD30 antigen found on the surface of some Hodgkin lymphoma cells) •      Histone deacetylase inhibitors (e.g., panobinostat or vorinostat, also known as Zolinza) •      Proteasome inhibitors (e.g., bortezomib, also known as Velcade) •      Alkylating agents (e.g., bendamustine, also known as Treanda)	topic_ll
74687	2	355457	5	NULL	NULL	0	NULL	SGN-35	GP		is a type of					monoclonal antibody	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Many promising therapies are currently under investigation in clinical trials for Hodgkin lymphoma. Types of therapy under investigation include: •      Monoclonal antibodies (e.g., SGN-35, which targets the CD30 antigen found on the surface of some Hodgkin lymphoma cells) •      Histone deacetylase inhibitors (e.g., panobinostat or vorinostat, also known as Zolinza) •      Proteasome inhibitors (e.g., bortezomib, also known as Velcade) •      Alkylating agents (e.g., bendamustine, also known as Treanda)	topic_ll
74688	3	355457	5	NULL	NULL	0	NULL	SGN-35	GP		targets					CD30 antigen	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Many promising therapies are currently under investigation in clinical trials for Hodgkin lymphoma. Types of therapy under investigation include: •      Monoclonal antibodies (e.g., SGN-35, which targets the CD30 antigen found on the surface of some Hodgkin lymphoma cells) •      Histone deacetylase inhibitors (e.g., panobinostat or vorinostat, also known as Zolinza) •      Proteasome inhibitors (e.g., bortezomib, also known as Velcade) •      Alkylating agents (e.g., bendamustine, also known as Treanda)	topic_ll
74689	4	355457	5	NULL	NULL	0	NULL	CD30 antigen	GP		is present in					Hodgkin lymphoma cells	Cell	surface of			NULL		0	NULL	NULL	NULL	NULL	NULL	Many promising therapies are currently under investigation in clinical trials for Hodgkin lymphoma. Types of therapy under investigation include: •      Monoclonal antibodies (e.g., SGN-35, which targets the CD30 antigen found on the surface of some Hodgkin lymphoma cells) •      Histone deacetylase inhibitors (e.g., panobinostat or vorinostat, also known as Zolinza) •      Proteasome inhibitors (e.g., bortezomib, also known as Velcade) •      Alkylating agents (e.g., bendamustine, also known as Treanda)	topic_ll
74690	5	355457	5	NULL	NULL	0	NULL	histone deacetylase inhibitors	Chemical		is used to treat		possibly			Hodgkin lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Many promising therapies are currently under investigation in clinical trials for Hodgkin lymphoma. Types of therapy under investigation include: •      Monoclonal antibodies (e.g., SGN-35, which targets the CD30 antigen found on the surface of some Hodgkin lymphoma cells) •      Histone deacetylase inhibitors (e.g., panobinostat or vorinostat, also known as Zolinza) •      Proteasome inhibitors (e.g., bortezomib, also known as Velcade) •      Alkylating agents (e.g., bendamustine, also known as Treanda)	topic_ll
74691	6	355457	5	NULL	NULL	0	NULL	panobinostat	Chemical		is a type of					histone deacetylase inhibitor	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Many promising therapies are currently under investigation in clinical trials for Hodgkin lymphoma. Types of therapy under investigation include: •      Monoclonal antibodies (e.g., SGN-35, which targets the CD30 antigen found on the surface of some Hodgkin lymphoma cells) •      Histone deacetylase inhibitors (e.g., panobinostat or vorinostat, also known as Zolinza) •      Proteasome inhibitors (e.g., bortezomib, also known as Velcade) •      Alkylating agents (e.g., bendamustine, also known as Treanda)	topic_ll
74692	7	355457	5	NULL	NULL	0	NULL	vorinostat	Chemical		is a type of					histone deacetylase inhibitor	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Many promising therapies are currently under investigation in clinical trials for Hodgkin lymphoma. Types of therapy under investigation include: •      Monoclonal antibodies (e.g., SGN-35, which targets the CD30 antigen found on the surface of some Hodgkin lymphoma cells) •      Histone deacetylase inhibitors (e.g., panobinostat or vorinostat, also known as Zolinza) •      Proteasome inhibitors (e.g., bortezomib, also known as Velcade) •      Alkylating agents (e.g., bendamustine, also known as Treanda)	topic_ll
74693	8	355457	5	NULL	NULL	0	NULL	vorinostat	Chemical		is known as					Zolinza	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Many promising therapies are currently under investigation in clinical trials for Hodgkin lymphoma. Types of therapy under investigation include: •      Monoclonal antibodies (e.g., SGN-35, which targets the CD30 antigen found on the surface of some Hodgkin lymphoma cells) •      Histone deacetylase inhibitors (e.g., panobinostat or vorinostat, also known as Zolinza) •      Proteasome inhibitors (e.g., bortezomib, also known as Velcade) •      Alkylating agents (e.g., bendamustine, also known as Treanda)	topic_ll
74694	9	355457	5	NULL	NULL	0	NULL	proteasome inhibitors	Chemical		is used to treat		possibly			Hodgkin lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Many promising therapies are currently under investigation in clinical trials for Hodgkin lymphoma. Types of therapy under investigation include: •      Monoclonal antibodies (e.g., SGN-35, which targets the CD30 antigen found on the surface of some Hodgkin lymphoma cells) •      Histone deacetylase inhibitors (e.g., panobinostat or vorinostat, also known as Zolinza) •      Proteasome inhibitors (e.g., bortezomib, also known as Velcade) •      Alkylating agents (e.g., bendamustine, also known as Treanda)	topic_ll
74695	10	355457	5	NULL	NULL	0	NULL	bortezomib	Chemical		is a type of					proteasome inhibitors	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Many promising therapies are currently under investigation in clinical trials for Hodgkin lymphoma. Types of therapy under investigation include: •      Monoclonal antibodies (e.g., SGN-35, which targets the CD30 antigen found on the surface of some Hodgkin lymphoma cells) •      Histone deacetylase inhibitors (e.g., panobinostat or vorinostat, also known as Zolinza) •      Proteasome inhibitors (e.g., bortezomib, also known as Velcade) •      Alkylating agents (e.g., bendamustine, also known as Treanda)	topic_ll
74696	11	355457	5	NULL	NULL	0	NULL	bortezomib	Chemical		is known as					Velcade	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Many promising therapies are currently under investigation in clinical trials for Hodgkin lymphoma. Types of therapy under investigation include: •      Monoclonal antibodies (e.g., SGN-35, which targets the CD30 antigen found on the surface of some Hodgkin lymphoma cells) •      Histone deacetylase inhibitors (e.g., panobinostat or vorinostat, also known as Zolinza) •      Proteasome inhibitors (e.g., bortezomib, also known as Velcade) •      Alkylating agents (e.g., bendamustine, also known as Treanda)	topic_ll
74697	12	355457	5	NULL	NULL	0	NULL	alkylating agents	Chemical		is used to treat		possibly			Hodgkin lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Many promising therapies are currently under investigation in clinical trials for Hodgkin lymphoma. Types of therapy under investigation include: •      Monoclonal antibodies (e.g., SGN-35, which targets the CD30 antigen found on the surface of some Hodgkin lymphoma cells) •      Histone deacetylase inhibitors (e.g., panobinostat or vorinostat, also known as Zolinza) •      Proteasome inhibitors (e.g., bortezomib, also known as Velcade) •      Alkylating agents (e.g., bendamustine, also known as Treanda)	topic_ll
74698	13	355457	5	NULL	NULL	0	NULL	bendamustine	Chemical		is a type of					alkylating agents	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Many promising therapies are currently under investigation in clinical trials for Hodgkin lymphoma. Types of therapy under investigation include: •      Monoclonal antibodies (e.g., SGN-35, which targets the CD30 antigen found on the surface of some Hodgkin lymphoma cells) •      Histone deacetylase inhibitors (e.g., panobinostat or vorinostat, also known as Zolinza) •      Proteasome inhibitors (e.g., bortezomib, also known as Velcade) •      Alkylating agents (e.g., bendamustine, also known as Treanda)	topic_ll
74699	14	355457	5	NULL	NULL	0	NULL	bendamustine	Chemical		is known as					Treanda	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Many promising therapies are currently under investigation in clinical trials for Hodgkin lymphoma. Types of therapy under investigation include: •      Monoclonal antibodies (e.g., SGN-35, which targets the CD30 antigen found on the surface of some Hodgkin lymphoma cells) •      Histone deacetylase inhibitors (e.g., panobinostat or vorinostat, also known as Zolinza) •      Proteasome inhibitors (e.g., bortezomib, also known as Velcade) •      Alkylating agents (e.g., bendamustine, also known as Treanda)	topic_ll
74700	1	355458	5	NULL	NULL	0	NULL	alkylating agents	Chemical		is used to treat		possibly			Hodgkin lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Many promising therapies are currently under investigation in clinical trials for Hodgkin lymphoma. Types of therapy under investigation include: •      Alkylating agents (e.g., bendamustine, also known as Treanda)	topic_ll
74701	2	355458	5	NULL	NULL	0	NULL	bendamustine	Chemical		is a type of					alkylating agents	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Many promising therapies are currently under investigation in clinical trials for Hodgkin lymphoma. Types of therapy under investigation include: •      Alkylating agents (e.g., bendamustine, also known as Treanda)	topic_ll
74702	3	355458	5	NULL	NULL	0	NULL	bendamustine	Chemical		is known as					Treanda	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Many promising therapies are currently under investigation in clinical trials for Hodgkin lymphoma. Types of therapy under investigation include: •      Alkylating agents (e.g., bendamustine, also known as Treanda)	topic_ll
74703	1	355459	5	NULL	NULL	0	NULL	HIV/AIDS	MedicalFinding		compromise on					immune system	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Having a compromised immune system, such as from HIV/AIDS or from having an organ transplant requiring medications to suppress your immune response, also appears to put you at a greater risk of Hodgkin's lymphoma	topic_ll
74704	2	355459	5	NULL	NULL	0	NULL	medications	Chemical		suppress					immune system	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Having a compromised immune system, such as from HIV/AIDS or from having an organ transplant requiring medications to suppress your immune response, also appears to put you at a greater risk of Hodgkin's lymphoma	topic_ll
74705	3	355459	5	NULL	NULL	0	NULL	organ transplant	MedicalProcedure		requires					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Having a compromised immune system, such as from HIV/AIDS or from having an organ transplant requiring medications to suppress your immune response, also appears to put you at a greater risk of Hodgkin's lymphoma	topic_ll
74706	4	355459	5	NULL	NULL	NULL	NULL	statement 1	Process		is at risk of		greater			Hodgkin lymphoma	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Having a compromised immune system, such as from HIV/AIDS or from having an organ transplant requiring medications to suppress your immune response, also appears to put you at a greater risk of Hodgkin's lymphoma	topic_ll
74707	5	355459	5	NULL	NULL	NULL	NULL	statement 3	Process		is at risk of		greater			Hodgkin lymphoma	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Having a compromised immune system, such as from HIV/AIDS or from having an organ transplant requiring medications to suppress your immune response, also appears to put you at a greater risk of Hodgkin's lymphoma	topic_ll
74708	1	355460	5	NULL	NULL	0	NULL	follicular lymphoma	MedicalFinding		is slow-growing		most common			NHL	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Slow-Growing or Indolent NHL * Follicular lymphoma - the most common slow-growing NHL * Chronic lymphocytic leukemia * Cutaneous T-cell lymphoma * Lymphoplasmacytic lymphoma * Marginal zone lymphoma * Mucosa-associated lymphoid tissue (MALT) lymphoma * Small cell lymphocytic lymphoma * Waldenström macroglobulinemia	topic_ll
74709	1	355461	5	NULL	NULL	NULL	NULL	Rituxan®	Chemical		is also known as					rituximab	Chemical				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Rituxan® (rituximab) and certain other drugs are used to treat some types of NHL	topic_ll
74710	2	355461	5	NULL	NULL	0	NULL	Rituxan®	Chemical		is used to treat					NHL	MedicalFinding	some types of			NULL		0	NULL	NULL	NULL	NULL	NULL	Rituxan® (rituximab) and certain other drugs are used to treat some types of NHL	topic_ll
74711	1	355464	5	NULL	NULL	0	NULL	Aranesp®	Chemical		increases					red cell	Cell	count of			NULL		0	NULL	NULL	NULL	NULL	NULL	Aranesp® (darbepoetin alfa) and Procrit® (epoetin alfa) - these can increase the red cell count 	topic_ll
74712	2	355464	5	NULL	NULL	0	NULL	Procrit®	Chemical		increases					red cell	Cell	count of			NULL		0	NULL	NULL	NULL	NULL	NULL	Aranesp® (darbepoetin alfa) and Procrit® (epoetin alfa) - these can increase the red cell count 	topic_ll
74713	3	355464	5	NULL	NULL	0	NULL	Procrit®	Chemical		is also known as					epoetin alfa	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Aranesp® (darbepoetin alfa) and Procrit® (epoetin alfa) - these can increase the red cell count 	topic_ll
74714	4	355464	5	NULL	NULL	0	NULL	Aranesp®	Chemical		is also known as					darbepoetin alfa	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Aranesp® (darbepoetin alfa) and Procrit® (epoetin alfa) - these can increase the red cell count 	topic_ll
74715	1	355465	5	NULL	NULL	0	NULL	Neupogen®	Chemical		is a synonym of					Neulasta®	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Neupogen® or Neulasta®(also called G-CSF ) and Leukine®(also called GM-CSF) - these can increase the number of neutrophils (white cells).	topic_ll
74716	2	355465	5	NULL	NULL	0	NULL	Neulasta®	Chemical		is also known as					G-CSF	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Neupogen® or Neulasta®(also called G-CSF ) and Leukine®(also called GM-CSF) - these can increase the number of neutrophils (white cells).	topic_ll
74717	3	355465	5	NULL	NULL	0	NULL	Leukine®	Chemical		is also known as					GM-CSF	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Neupogen® or Neulasta®(also called G-CSF ) and Leukine®(also called GM-CSF) - these can increase the number of neutrophils (white cells).	topic_ll
74718	4	355465	5	NULL	NULL	0	NULL	Leukine®	Chemical		increases					neutrophils	Cell	number of			NULL		0	NULL	NULL	NULL	NULL	NULL	Neupogen® or Neulasta®(also called G-CSF ) and Leukine®(also called GM-CSF) - these can increase the number of neutrophils (white cells).	topic_ll
74719	5	355465	5	NULL	NULL	0	NULL	Neulasta®	Chemical		increases					neutrophils	Cell	number of			NULL		0	NULL	NULL	NULL	NULL	NULL	Neupogen® or Neulasta®(also called G-CSF ) and Leukine®(also called GM-CSF) - these can increase the number of neutrophils (white cells).	topic_ll
74720	6	355465	5	NULL	NULL	0	NULL	neutrophils	Cell		is a type of					white cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Neupogen® or Neulasta®(also called G-CSF ) and Leukine®(also called GM-CSF) - these can increase the number of neutrophils (white cells).	topic_ll
74778	1	355466	5	NULL	NULL	0	NULL	Neupogen®	Chemical		is a synonym of					Neulasta®	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	A red cell transfusion or drugs called blood cell growth factors may be needed until the side effects of chemotherapy wear off. Neupogen® or Neulasta®(also called G-CSF ) and Leukine®(also called GM-CSF) - these can increase the number of neutrophils (white cells).	topic_ll
74779	2	355466	5	NULL	NULL	0	NULL	Neulasta®	Chemical		is also known as					G-CSF	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	A red cell transfusion or drugs called blood cell growth factors may be needed until the side effects of chemotherapy wear off. Neupogen® or Neulasta®(also called G-CSF ) and Leukine®(also called GM-CSF) - these can increase the number of neutrophils (white cells).	topic_ll
74780	3	355466	5	NULL	NULL	0	NULL	Leukine®	Chemical		is also known as					GM-CSF	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	A red cell transfusion or drugs called blood cell growth factors may be needed until the side effects of chemotherapy wear off. Neupogen® or Neulasta®(also called G-CSF ) and Leukine®(also called GM-CSF) - these can increase the number of neutrophils (white cells).	topic_ll
74781	4	355466	5	NULL	NULL	NULL	NULL	Neulasta®	Chemical		increases					neutrophils	Cell	number of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	A red cell transfusion or drugs called blood cell growth factors may be needed until the side effects of chemotherapy wear off. Neupogen® or Neulasta®(also called G-CSF ) and Leukine®(also called GM-CSF) - these can increase the number of neutrophils (white cells).	topic_ll
74782	5	355466	5	NULL	NULL	NULL	NULL	Leukine®	Chemical		increases					neutrophils	Cell	number of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	A red cell transfusion or drugs called blood cell growth factors may be needed until the side effects of chemotherapy wear off. Neupogen® or Neulasta®(also called G-CSF ) and Leukine®(also called GM-CSF) - these can increase the number of neutrophils (white cells).	topic_ll
74783	6	355466	5	NULL	NULL	0	NULL	neutrophils	Cell		is a type of					white cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	A red cell transfusion or drugs called blood cell growth factors may be needed until the side effects of chemotherapy wear off. Neupogen® or Neulasta®(also called G-CSF ) and Leukine®(also called GM-CSF) - these can increase the number of neutrophils (white cells).	topic_ll
74784	1	355467	5	NULL	NULL	0	NULL	Aranesp®	Chemical		is also known as					Darbepoetin alfa	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	A red cell transfusion or drugs called blood cell growth factors may be needed until the side effects of chemotherapy wear off. Aranesp® (Darbepoetin alfa) and Procrit® (epoetin alfa) - these can increase the red cell count 	topic_ll
74785	2	355467	5	NULL	NULL	0	NULL	Procrit®	Chemical		is also known as					epoetin alfa	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	A red cell transfusion or drugs called blood cell growth factors may be needed until the side effects of chemotherapy wear off. Aranesp® (Darbepoetin alfa) and Procrit® (epoetin alfa) - these can increase the red cell count 	topic_ll
74786	3	355467	5	NULL	NULL	0	NULL	Procrit®	Chemical		induce					red cell	Cell	count of			NULL		0	NULL	NULL	NULL	NULL	NULL	A red cell transfusion or drugs called blood cell growth factors may be needed until the side effects of chemotherapy wear off. Aranesp® (Darbepoetin alfa) and Procrit® (epoetin alfa) - these can increase the red cell count 	topic_ll
74787	4	355467	5	NULL	NULL	0	NULL	Aranesp®	Chemical		increases					red cell	Cell	count of			NULL		0	NULL	NULL	NULL	NULL	NULL	A red cell transfusion or drugs called blood cell growth factors may be needed until the side effects of chemotherapy wear off. Aranesp® (Darbepoetin alfa) and Procrit® (epoetin alfa) - these can increase the red cell count 	topic_ll
75927	1	355468	7	NULL	NULL	0	NULL	pregnant women	GroupOfPeople		likely to have					depression	MedicalFinding	diagnosis of			NULL		0	NULL	NULL	NULL	NULL	NULL	this cohort study of more than 43,000 women from the Veterans Health Administration system found that those who were pregnant were twice as likely to have a diagnosis of depression, anxiety, posttraumatic stress disorder (PTSD), bipolar disorder, or schizophrenia as their counterparts who were not pregnant.	topic_bd
75928	2	355468	7	NULL	NULL	0	NULL	pregnant women	GroupOfPeople		likely to have					anxiety	MedicalFinding	diagnosis of			NULL		0	NULL	NULL	NULL	NULL	NULL	this cohort study of more than 43,000 women from the Veterans Health Administration system found that those who were pregnant were twice as likely to have a diagnosis of depression, anxiety, posttraumatic stress disorder (PTSD), bipolar disorder, or schizophrenia as their counterparts who were not pregnant.	topic_bd
75929	3	355468	7	NULL	NULL	0	NULL	pregnant women	GroupOfPeople		likely to have					PTSD	MedicalFinding	diagnosis of			NULL		0	NULL	NULL	NULL	NULL	NULL	this cohort study of more than 43,000 women from the Veterans Health Administration system found that those who were pregnant were twice as likely to have a diagnosis of depression, anxiety, posttraumatic stress disorder (PTSD), bipolar disorder, or schizophrenia as their counterparts who were not pregnant.	topic_bd
75930	4	355468	7	NULL	NULL	0	NULL	pregnant women	GroupOfPeople		likely to have					bipolar disorder	MedicalFinding	diagnosis of			NULL		0	NULL	NULL	NULL	NULL	NULL	this cohort study of more than 43,000 women from the Veterans Health Administration system found that those who were pregnant were twice as likely to have a diagnosis of depression, anxiety, posttraumatic stress disorder (PTSD), bipolar disorder, or schizophrenia as their counterparts who were not pregnant.	topic_bd
75931	5	355468	7	NULL	NULL	0	NULL	pregnant women	GroupOfPeople		likely to have					schizophrenia	MedicalFinding	diagnosis of			NULL		0	NULL	NULL	NULL	NULL	NULL	this cohort study of more than 43,000 women from the Veterans Health Administration system found that those who were pregnant were twice as likely to have a diagnosis of depression, anxiety, posttraumatic stress disorder (PTSD), bipolar disorder, or schizophrenia as their counterparts who were not pregnant.	topic_bd
75932	6	355468	7	NULL	NULL	0	NULL	PTSD	MedicalFinding		is					posttraumatic stress disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	this cohort study of more than 43,000 women from the Veterans Health Administration system found that those who were pregnant were twice as likely to have a diagnosis of depression, anxiety, posttraumatic stress disorder (PTSD), bipolar disorder, or schizophrenia as their counterparts who were not pregnant.	topic_bd
75933	7	355468	7	NULL	NULL	0	NULL	nonpregnant women	GroupOfPeople		likely to have					depression	MedicalFinding	diagnosis of			NULL		0	NULL	NULL	NULL	NULL	NULL	this cohort study of more than 43,000 women from the Veterans Health Administration system found that those who were pregnant were twice as likely to have a diagnosis of depression, anxiety, posttraumatic stress disorder (PTSD), bipolar disorder, or schizophrenia as their counterparts who were not pregnant.	topic_bd
75934	8	355468	7	NULL	NULL	0	NULL	nonpregnant women	GroupOfPeople		likely to have					anxiety	MedicalFinding	diagnosis of			NULL		0	NULL	NULL	NULL	NULL	NULL	this cohort study of more than 43,000 women from the Veterans Health Administration system found that those who were pregnant were twice as likely to have a diagnosis of depression, anxiety, posttraumatic stress disorder (PTSD), bipolar disorder, or schizophrenia as their counterparts who were not pregnant.	topic_bd
75935	9	355468	7	NULL	NULL	0	NULL	nonpregnant women	GroupOfPeople		likely to have					PTSD	MedicalFinding	diagnosis of			NULL		0	NULL	NULL	NULL	NULL	NULL	this cohort study of more than 43,000 women from the Veterans Health Administration system found that those who were pregnant were twice as likely to have a diagnosis of depression, anxiety, posttraumatic stress disorder (PTSD), bipolar disorder, or schizophrenia as their counterparts who were not pregnant.	topic_bd
75936	10	355468	7	NULL	NULL	0	NULL	nonpregnant women	GroupOfPeople		likely to have					bipolar disorder	MedicalFinding	diagnosis of			NULL		0	NULL	NULL	NULL	NULL	NULL	this cohort study of more than 43,000 women from the Veterans Health Administration system found that those who were pregnant were twice as likely to have a diagnosis of depression, anxiety, posttraumatic stress disorder (PTSD), bipolar disorder, or schizophrenia as their counterparts who were not pregnant.	topic_bd
75937	11	355468	7	NULL	NULL	0	NULL	nonpregnant women	GroupOfPeople		likely to have					schizophrenia	MedicalFinding	diagnosis of			NULL		0	NULL	NULL	NULL	NULL	NULL	this cohort study of more than 43,000 women from the Veterans Health Administration system found that those who were pregnant were twice as likely to have a diagnosis of depression, anxiety, posttraumatic stress disorder (PTSD), bipolar disorder, or schizophrenia as their counterparts who were not pregnant.	topic_bd
75938	12	355468	7	NULL	NULL	0	NULL	statement 1	Process	occurence in	is more than					statement 7	Process	occurence in			NULL		0	NULL	NULL	NULL	NULL	NULL	this cohort study of more than 43,000 women from the Veterans Health Administration system found that those who were pregnant were twice as likely to have a diagnosis of depression, anxiety, posttraumatic stress disorder (PTSD), bipolar disorder, or schizophrenia as their counterparts who were not pregnant.	topic_bd
75939	13	355468	7	NULL	NULL	0	NULL	statement 2	Process	occurence in	is more than					statement 8	Process	occurence in			NULL		0	NULL	NULL	NULL	NULL	NULL	this cohort study of more than 43,000 women from the Veterans Health Administration system found that those who were pregnant were twice as likely to have a diagnosis of depression, anxiety, posttraumatic stress disorder (PTSD), bipolar disorder, or schizophrenia as their counterparts who were not pregnant.	topic_bd
75940	14	355468	7	NULL	NULL	0	NULL	statement 3	Process	occurence in	is more than					statement 9	Process	occurence in			NULL		0	NULL	NULL	NULL	NULL	NULL	this cohort study of more than 43,000 women from the Veterans Health Administration system found that those who were pregnant were twice as likely to have a diagnosis of depression, anxiety, posttraumatic stress disorder (PTSD), bipolar disorder, or schizophrenia as their counterparts who were not pregnant.	topic_bd
75941	15	355468	7	NULL	NULL	0	NULL	statement 4	Process	occurence in	is more than					statement 10	Process	occurence in			NULL		0	NULL	NULL	NULL	NULL	NULL	this cohort study of more than 43,000 women from the Veterans Health Administration system found that those who were pregnant were twice as likely to have a diagnosis of depression, anxiety, posttraumatic stress disorder (PTSD), bipolar disorder, or schizophrenia as their counterparts who were not pregnant.	topic_bd
75942	16	355468	7	NULL	NULL	0	NULL	statement 5	Process	occurence in	is more than					statement 11	Process	occurence in			NULL		0	NULL	NULL	NULL	NULL	NULL	this cohort study of more than 43,000 women from the Veterans Health Administration system found that those who were pregnant were twice as likely to have a diagnosis of depression, anxiety, posttraumatic stress disorder (PTSD), bipolar disorder, or schizophrenia as their counterparts who were not pregnant.	topic_bd
75943	1	355472	7	NULL	NULL	0	NULL	scholastic achievement	MentalProcess		is in relation with					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	the relationship between scholastic achievement and bipolar disorder appeared to be stronger in boys than girls.	topic_bd
75944	2	355472	7	NULL	NULL	0	NULL	statement 1	Process		appear in					boys	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	the relationship between scholastic achievement and bipolar disorder appeared to be stronger in boys than girls.	topic_bd
75945	3	355472	7	NULL	NULL	0	NULL	statement 2	Process		appear in					girls	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	the relationship between scholastic achievement and bipolar disorder appeared to be stronger in boys than girls.	topic_bd
75946	4	355472	7	NULL	NULL	0	NULL	statement 2	Process		more stronger than					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	the relationship between scholastic achievement and bipolar disorder appeared to be stronger in boys than girls.	topic_bd
75947	1	355473	7	NULL	NULL	0	NULL	creative people	GroupOfPeople		more susceptible to					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The study gives credence to the idea that creative people are more susceptible to bipolar disorder.	topic_bd
75948	1	355474	7	NULL	NULL	0	NULL	higher academic marks 	QuantityOrMeasure		associated with					schizophrenia	MedicalFinding	decreased risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	higher academic marks are associated with decreased risk for schizophrenia, the study authors noted.	topic_bd
75949	1	355475	7	NULL	NULL	0	NULL	schizophrenia 	MedicalFinding		genetically linked to		closely			bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	That’s "very striking" in light of a recent theory that schizophrenia and bipolar disorder are more closely genetically linked than previously believed, commented Dr. MacCabe. 	topic_bd
75950	1	355476	7	NULL	NULL	0	NULL	autoimmune thyroiditis	MedicalFinding		related to					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In a study of twins, autoimmune thyroiditis was related to bipolar disorder and the genetic tendency to develop bipolar disorder.	topic_bd
75951	2	355476	7	NULL	NULL	0	NULL	statement 1	Process		occur in					twins	Person				NULL		0	NULL	NULL	NULL	NULL	NULL	In a study of twins, autoimmune thyroiditis was related to bipolar disorder and the genetic tendency to develop bipolar disorder.	topic_bd
75952	3	355476	7	NULL	NULL	0	NULL	twins	Person		genetic tendency					bipolar disorder	MedicalFinding	to develop			NULL		0	NULL	NULL	NULL	NULL	NULL	In a study of twins, autoimmune thyroiditis was related to bipolar disorder and the genetic tendency to develop bipolar disorder.	topic_bd
75969	1	355477	7	NULL	NULL	NULL	NULL	Thyroid dysfunction	MedicalFinding		occur in					rapid cycling bipolar disorder	MedicalFinding	patients with			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Thyroid dysfunction is more common in patients with rapid cycling bipolar disorder (ie, having 4 or more mood swings or episodes in a 12-month period) or mixed states (ie, an episode that simultaneously presents symptoms of both depression and mania) than in patients with classic mania	topic_bd
75970	2	355477	7	NULL	NULL	0	NULL	Thyroid dysfunction	MedicalFinding		occur in					mixed state	MedicalFinding	patients with			NULL		0	NULL	NULL	NULL	NULL	NULL	Thyroid dysfunction is more common in patients with rapid cycling bipolar disorder (ie, having 4 or more mood swings or episodes in a 12-month period) or mixed states (ie, an episode that simultaneously presents symptoms of both depression and mania) than in patients with classic mania	topic_bd
75971	3	355477	7	NULL	NULL	0	NULL	Thyroid dysfunction	MedicalFinding		occur in					classic mania	MedicalFinding	patients with			NULL		0	NULL	NULL	NULL	NULL	NULL	Thyroid dysfunction is more common in patients with rapid cycling bipolar disorder (ie, having 4 or more mood swings or episodes in a 12-month period) or mixed states (ie, an episode that simultaneously presents symptoms of both depression and mania) than in patients with classic mania	topic_bd
75972	1	355478	7	NULL	NULL	0	NULL	Levothyroxine 	GP		decrease		may			manic episodes	MedicalFinding	severity of			NULL		0	NULL	NULL	NULL	NULL	NULL	Levothyroxine may decrease the severity and frequency of manic and depressive episodes.	topic_bd
75973	2	355478	7	NULL	NULL	NULL	NULL	Levothyroxine	GP		decrease		may			depressive episodes	MedicalFinding	severity of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Levothyroxine may decrease the severity and frequency of manic and depressive episodes.	topic_bd
75974	3	355478	7	NULL	NULL	0	NULL	Levothyroxine	GP		decrease		may			manic episodes	MedicalFinding	frequency of			NULL		0	NULL	NULL	NULL	NULL	NULL	Levothyroxine may decrease the severity and frequency of manic and depressive episodes.	topic_bd
75975	4	355478	7	NULL	NULL	NULL	NULL	Levothyroxine	GP		decrease		may			depressive episodes	MedicalFinding	frequency of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Levothyroxine may decrease the severity and frequency of manic and depressive episodes.	topic_bd
75976	1	355479	7	NULL	NULL	0	NULL	Levothyroxine	GP		is a synthetic form of					thyroxine	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Levothyroxine, also L-thyroxine, synthetic T4, or 3,5,3',5'-tetraiodo-L-thyronine, is a synthetic form of thyroxine (thyroid hormone), used as a hormone replacement for patients with thyroid problems.	topic_bd
75977	2	355479	7	NULL	NULL	0	NULL	L-thyroxine	GP		is a synthetic form of					thyroxine	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Levothyroxine, also L-thyroxine, synthetic T4, or 3,5,3',5'-tetraiodo-L-thyronine, is a synthetic form of thyroxine (thyroid hormone), used as a hormone replacement for patients with thyroid problems.	topic_bd
75978	3	355479	7	NULL	NULL	NULL	NULL	synthetic T4	GP		is a synthetic form of					thyroxine	GP				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Levothyroxine, also L-thyroxine, synthetic T4, or 3,5,3',5'-tetraiodo-L-thyronine, is a synthetic form of thyroxine (thyroid hormone), used as a hormone replacement for patients with thyroid problems.	topic_bd
75979	4	355479	7	NULL	NULL	0	NULL	3,5,3',5'-tetraiodo-L-thyronine	GP		is a synthetic form of					thyroxine	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Levothyroxine, also L-thyroxine, synthetic T4, or 3,5,3',5'-tetraiodo-L-thyronine, is a synthetic form of thyroxine (thyroid hormone), used as a hormone replacement for patients with thyroid problems.	topic_bd
75980	5	355479	7	NULL	NULL	0	NULL	statement 1	Process		used as					hormone	GP	replacement of			NULL		0	NULL	NULL	NULL	NULL	NULL	Levothyroxine, also L-thyroxine, synthetic T4, or 3,5,3',5'-tetraiodo-L-thyronine, is a synthetic form of thyroxine (thyroid hormone), used as a hormone replacement for patients with thyroid problems.	topic_bd
75981	6	355479	7	NULL	NULL	0	NULL	statement 2	Process		used as					hormone	GP	replacement of			NULL		0	NULL	NULL	NULL	NULL	NULL	Levothyroxine, also L-thyroxine, synthetic T4, or 3,5,3',5'-tetraiodo-L-thyronine, is a synthetic form of thyroxine (thyroid hormone), used as a hormone replacement for patients with thyroid problems.	topic_bd
75982	7	355479	7	NULL	NULL	0	NULL	statement 3	Process		used as					hormone	GP	replacement of			NULL		0	NULL	NULL	NULL	NULL	NULL	Levothyroxine, also L-thyroxine, synthetic T4, or 3,5,3',5'-tetraiodo-L-thyronine, is a synthetic form of thyroxine (thyroid hormone), used as a hormone replacement for patients with thyroid problems.	topic_bd
75983	8	355479	7	NULL	NULL	0	NULL	statement 4	Process		used as					hormone	GP	replacement of			NULL		0	NULL	NULL	NULL	NULL	NULL	Levothyroxine, also L-thyroxine, synthetic T4, or 3,5,3',5'-tetraiodo-L-thyronine, is a synthetic form of thyroxine (thyroid hormone), used as a hormone replacement for patients with thyroid problems.	topic_bd
75984	9	355479	7	NULL	NULL	0	NULL	thyroxine	GP		is					thyroid hormone	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Levothyroxine, also L-thyroxine, synthetic T4, or 3,5,3',5'-tetraiodo-L-thyronine, is a synthetic form of thyroxine (thyroid hormone), used as a hormone replacement for patients with thyroid problems.	topic_bd
75985	10	355479	7	NULL	NULL	0	NULL	statement 5	Process		occur in					thyroid patients	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Levothyroxine, also L-thyroxine, synthetic T4, or 3,5,3',5'-tetraiodo-L-thyronine, is a synthetic form of thyroxine (thyroid hormone), used as a hormone replacement for patients with thyroid problems.	topic_bd
75986	11	355479	7	NULL	NULL	0	NULL	statement 6	Process		occur in					thyroid patients	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Levothyroxine, also L-thyroxine, synthetic T4, or 3,5,3',5'-tetraiodo-L-thyronine, is a synthetic form of thyroxine (thyroid hormone), used as a hormone replacement for patients with thyroid problems.	topic_bd
75987	12	355479	7	NULL	NULL	0	NULL	statement 7	Process		occur in					thyroid patients	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Levothyroxine, also L-thyroxine, synthetic T4, or 3,5,3',5'-tetraiodo-L-thyronine, is a synthetic form of thyroxine (thyroid hormone), used as a hormone replacement for patients with thyroid problems.	topic_bd
75988	13	355479	7	NULL	NULL	0	NULL	statement 8	Process		occur in					thyroid patients	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Levothyroxine, also L-thyroxine, synthetic T4, or 3,5,3',5'-tetraiodo-L-thyronine, is a synthetic form of thyroxine (thyroid hormone), used as a hormone replacement for patients with thyroid problems.	topic_bd
75989	1	355480	7	NULL	NULL	0	NULL	triiodothyronine	GP		used as		effectively			augmentation agent	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	In addition, triiodothyronine has been effectively used as an augmentation agent in treatment-resistant bipolar depression.	topic_bd
75990	2	355480	7	NULL	NULL	0	NULL	statement 1	Process		is used in					treatment-resistant bipolar depression	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In addition, triiodothyronine has been effectively used as an augmentation agent in treatment-resistant bipolar depression.	topic_bd
75991	1	355481	7	NULL	NULL	NULL	NULL	Triiodothyronine	AminoAcid		also known as					T3	AminoAcid				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Triiodothyronine, C15H12I3NO4, also known as T3, is a thyroid hormone	topic_bd
75992	2	355481	7	NULL	NULL	0	NULL	T3	AminoAcid		is a type of					thyroid hormone	AminoAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	Triiodothyronine, C15H12I3NO4, also known as T3, is a thyroid hormone	topic_bd
75993	3	355481	7	NULL	NULL	0	NULL	C15H12I3NO4	AminoAcid		also known as					T3	AminoAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	Triiodothyronine, C15H12I3NO4, also known as T3, is a thyroid hormone	topic_bd
75994	1	355482	7	NULL	NULL	0	NULL	bipolar disorder patients	MedicalFinding		greater risk for					hyperthyroidism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In a Danish registry study,[7] patients hospitalized with bipolar disorder were at greater risk for readmission with hyperthyroidism compared with control patients. 	topic_bd
75995	1	355483	7	NULL	NULL	0	NULL	 mania	MedicalFinding		associated with					hypothyroidism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	there are case reports of mania or hypomania associated with hypothyroidism. 	topic_bd
75996	2	355483	7	NULL	NULL	0	NULL	hypomania	MedicalFinding		associated with					hypothyroidism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	there are case reports of mania or hypomania associated with hypothyroidism. 	topic_bd
75997	3	355483	7	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	there are case reports of mania or hypomania associated with hypothyroidism. 	topic_bd
76042	1	355484	7	NULL	NULL	NULL	NULL	free thyroxine index 	GP	lower values of	associated with					bipolar depression	MedicalFinding	longer time to remission in patients with			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cole and colleagues[9] evaluated free thyroxine index and thyroid-stimulating hormone (TSH) levels in 65 patients with bipolar depression. A longer time to remission was significantly associated with both lower values of free thyroxine index and higher values of TSH.	topic_bd
76043	2	355484	7	NULL	NULL	0	NULL	TSH	GP	higher values of	associated with					bipolar depression	MedicalFinding	longer time to remission in patients with			NULL		0	NULL	NULL	NULL	NULL	NULL	Cole and colleagues[9] evaluated free thyroxine index and thyroid-stimulating hormone (TSH) levels in 65 patients with bipolar depression. A longer time to remission was significantly associated with both lower values of free thyroxine index and higher values of TSH.	topic_bd
76044	1	355485	7	NULL	NULL	0	NULL	Hypothyroidism 	MedicalFinding		occur upon		may			lithium	Chemical	use of			NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothyroidism may occur in the early years of lithium use, in middle-aged women, and when thyroid autoimmunity is present;	topic_bd
76045	2	355485	7	NULL	NULL	0	NULL	statement 1	Process		occur in					middle-aged women	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothyroidism may occur in the early years of lithium use, in middle-aged women, and when thyroid autoimmunity is present;	topic_bd
76046	3	355485	7	NULL	NULL	0	NULL	statement 1	Process		occur upon					thyroid autoimmunity	MedicalFinding	presence of			NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothyroidism may occur in the early years of lithium use, in middle-aged women, and when thyroid autoimmunity is present;	topic_bd
76047	1	355486	7	NULL	NULL	0	NULL	Hyperthyroidism	MedicalFinding		uncommon during					lithium	Chemical	treatment with			NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperthyroidism and thyroid cancer are uncommon during treatment with lithium.	topic_bd
76048	2	355486	7	NULL	NULL	0	NULL	thyroid cancer	MedicalFinding		uncommon during					lithium	Chemical	treatment with			NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperthyroidism and thyroid cancer are uncommon during treatment with lithium.	topic_bd
76049	1	355487	7	NULL	NULL	0	NULL	thyroid dysfunction 	MedicalFinding	lithium treated	is not different from					general population	GroupOfPeople	observed in			NULL		0	NULL	NULL	NULL	NULL	NULL	The outcome of thyroid dysfunction in patients who have been on lithium for many years is not greatly different from that observed in the general population	topic_bd
76050	1	355488	7	NULL	NULL	0	NULL	Classic bipolar disorder	MedicalFinding		have difficulty					face emotions	MentalProcess	labeling			NULL		0	NULL	NULL	NULL	NULL	NULL	Earlier research had shown that both youth with classic, episodic bipolar and those with nonepisodic irritability have difficulty labeling face emotions.	topic_bd
76051	2	355488	7	NULL	NULL	0	NULL	episodic bipolar disorder	MedicalFinding		have difficulty					face emotions	MentalProcess	labeling			NULL		0	NULL	NULL	NULL	NULL	NULL	Earlier research had shown that both youth with classic, episodic bipolar and those with nonepisodic irritability have difficulty labeling face emotions.	topic_bd
76052	3	355488	7	NULL	NULL	0	NULL	nonepisodic irritability 	MedicalFinding		have difficulty					face emotions	MentalProcess	labeling			NULL		0	NULL	NULL	NULL	NULL	NULL	Earlier research had shown that both youth with classic, episodic bipolar and those with nonepisodic irritability have difficulty labeling face emotions.	topic_bd
76248	1	355489	7	NULL	NULL	0	NULL	healthy subjects	GroupOfPeople	amygdala activation  in	does not differ from		significantly			bipolar disorder	MedicalFinding	amygdala activation in patients with			NULL		0	NULL	NULL	NULL	NULL	NULL	, the study shows that patients with bipolar disorder did not differ significantly from healthy comparison subjects in amygdala activation. 	topic_bd
76249	1	355518	7	NULL	NULL	0	NULL	Alcohol 	Chemical	misuse of	associated with					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Alcohol misuse is associated with bipolar disorder.	topic_bd
76250	1	355519	7	NULL	NULL	0	NULL	circadian clockwork	Process	abnormalities in	play a role in					bipolar disorder	MedicalFinding	pathogenesis of			NULL		0	NULL	NULL	NULL	NULL	NULL	Abnormalities in the circadian clockwork play a role in the pathogenesis of bipolar disorder	topic_bd
76251	1	355520	7	NULL	NULL	0	NULL	Alcohol 	Chemical	intake of	affect		likely			circadian phenotype	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	NULL	NULL	Alcohol intake is likely to affect the circadian phenotype.	topic_bd
76252	1	355521	7	NULL	NULL	NULL	NULL	co-morbid alcohol use disorder patients	GroupOfPeople		were more of					morning type	Time				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patients with the co-morbid alcohol use disorder were more of the morning type as compared with patients with bipolar disorder only.	topic_bd
76253	2	355521	7	NULL	NULL	0	NULL	statement 1	Process		in comparison with					bipolar disorder patients	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with the co-morbid alcohol use disorder were more of the morning type as compared with patients with bipolar disorder only.	topic_bd
76254	1	355522	7	NULL	NULL	0	NULL	Co-morbid patients	GroupOfPeople		prefers					daily activities	Process	morning hours			NULL		0	NULL	NULL	NULL	NULL	NULL	Co-morbid patients preferred more the morning hours for their daily activities, indicative of alcohol consumption having an effect on the circadian clock.	topic_bd
76255	2	355522	7	NULL	NULL	NULL	NULL	statement 1	Process		indicates					alcohol 	Process	consumption of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Co-morbid patients preferred more the morning hours for their daily activities, indicative of alcohol consumption having an effect on the circadian clock.	topic_bd
76256	3	355522	7	NULL	NULL	0	NULL	statement 2	Process		effect					circadian clock	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Co-morbid patients preferred more the morning hours for their daily activities, indicative of alcohol consumption having an effect on the circadian clock.	topic_bd
76257	1	355523	7	NULL	NULL	NULL	NULL	sleep deprivation	MedicalFinding		alleviate					depression	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	sleep deprivation tends to alleviate depression in patients with bipolar disorder 	topic_bd
76258	2	355523	7	NULL	NULL	0	NULL	statement 1	Process		in patients with					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	sleep deprivation tends to alleviate depression in patients with bipolar disorder 	topic_bd
76259	1	355524	7	NULL	NULL	0	NULL	Lithium	Chemical		acts on		directly			circadian pacemaker cells 	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Lithium acts directly on the circadian pacemaker cells and lengthens the period of circadian rhythms	topic_bd
76260	2	355524	7	NULL	NULL	0	NULL	statement 1	Process		lengthens					circadian rhythms	Process	period of			NULL		0	NULL	NULL	NULL	NULL	NULL	Lithium acts directly on the circadian pacemaker cells and lengthens the period of circadian rhythms	topic_bd
76261	1	355525	7	NULL	NULL	NULL	NULL	bipolar disorder	MedicalFinding	Preschool children of parents with	is in the risk of					ADHD	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Preschool children of parents with bipolar disorder have more than an 8-fold higher risk for attention-deficit/hyperactivity disorder (ADHD) than offspring of parents without this disorder	topic_bd
76262	2	355525	7	NULL	NULL	NULL	NULL	bipolar disorder	MedicalFinding	Preschool children of parents without	is in the risk of					ADHD	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Preschool children of parents with bipolar disorder have more than an 8-fold higher risk for attention-deficit/hyperactivity disorder (ADHD) than offspring of parents without this disorder	topic_bd
76263	3	355525	7	NULL	NULL	NULL	NULL	statement 1	Process	risk of	is higher than					statement 2	Process	risk of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Preschool children of parents with bipolar disorder have more than an 8-fold higher risk for attention-deficit/hyperactivity disorder (ADHD) than offspring of parents without this disorder	topic_bd
76268	4	355525	7	NULL	NULL	0	NULL	ADHD	MedicalFinding		is					attention-deficit/hyperactivity disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Preschool children of parents with bipolar disorder have more than an 8-fold higher risk for attention-deficit/hyperactivity disorder (ADHD) than offspring of parents without this disorder	topic_bd
76264	1	355526	7	NULL	NULL	0	NULL	suicide	MentalProcess	 risk of	is increased in					bipolar disorder	MedicalFinding	patients with			NULL		0	NULL	NULL	NULL	NULL	NULL	Clinicians should know that, on average in the United States, 1 suicide occurs for every 30 attempts. In bipolar patients, it's 1 suicide for every 3 attempts,[1] which confirms the increased risk of suicide in patients with bipolar disorder: their attempts are 10 times more lethal.	topic_bd
76265	1	355527	7	NULL	NULL	0	NULL	Suicide	MentalProcess		outcome of		devastating			depression	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Suicide is a devastating outcome of depression, and patients with bipolar disorder spend more time depressed than manic.	topic_bd
76266	2	355527	7	NULL	NULL	NULL	NULL	bipolar disorder	MedicalFinding	depression in patients with	is more than					bipolar disorder	MedicalFinding	manic in patients with			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Suicide is a devastating outcome of depression, and patients with bipolar disorder spend more time depressed than manic.	topic_bd
76267	1	355528	7	NULL	NULL	0	NULL	Bipolar patients	MedicalFinding		have					mixed mood states	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar patients sometimes have mixed mood states, in which they're both depressed and manic at the same time. In other words, they're not euphoric like most manic patients, they're irritable and they have increased energy. That's a particularly risky situation for a bipolar patient.	topic_bd
76269	2	355528	7	NULL	NULL	NULL	NULL	depression	MedicalFinding		occur at the same time as					manic	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bipolar patients sometimes have mixed mood states, in which they're both depressed and manic at the same time. In other words, they're not euphoric like most manic patients, they're irritable and they have increased energy. That's a particularly risky situation for a bipolar patient.	topic_bd
76270	3	355528	7	NULL	NULL	0	NULL	statement 2	Process		occur in					bipolar patients	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar patients sometimes have mixed mood states, in which they're both depressed and manic at the same time. In other words, they're not euphoric like most manic patients, they're irritable and they have increased energy. That's a particularly risky situation for a bipolar patient.	topic_bd
76271	4	355528	7	NULL	NULL	0	NULL	Bipolar patients	MedicalFinding		are not					euphoric	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar patients sometimes have mixed mood states, in which they're both depressed and manic at the same time. In other words, they're not euphoric like most manic patients, they're irritable and they have increased energy. That's a particularly risky situation for a bipolar patient.	topic_bd
76272	5	355528	7	NULL	NULL	0	NULL	manic patients	MedicalFinding		are					euphoric	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar patients sometimes have mixed mood states, in which they're both depressed and manic at the same time. In other words, they're not euphoric like most manic patients, they're irritable and they have increased energy. That's a particularly risky situation for a bipolar patient.	topic_bd
76273	6	355528	7	NULL	NULL	0	NULL	Bipolar patients	MedicalFinding		are					irritable	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar patients sometimes have mixed mood states, in which they're both depressed and manic at the same time. In other words, they're not euphoric like most manic patients, they're irritable and they have increased energy. That's a particularly risky situation for a bipolar patient.	topic_bd
76274	7	355528	7	NULL	NULL	0	NULL	Bipolar patients	MedicalFinding		have increased					energy	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar patients sometimes have mixed mood states, in which they're both depressed and manic at the same time. In other words, they're not euphoric like most manic patients, they're irritable and they have increased energy. That's a particularly risky situation for a bipolar patient.	topic_bd
76275	8	355528	7	NULL	NULL	0	NULL	statement 1	Process		risky situation for					bipolar patient	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar patients sometimes have mixed mood states, in which they're both depressed and manic at the same time. In other words, they're not euphoric like most manic patients, they're irritable and they have increased energy. That's a particularly risky situation for a bipolar patient.	topic_bd
76327	1	355529	7	NULL	NULL	NULL	NULL	severe anxiety	MedicalFinding		risk factor for					suicide	MentalProcess				NULL		NULL	NULL	NULL	NULL	NULL	NULL	if the patient is experiencing severe anxiety, such as anxious thoughts the patient can't stop. This could be a serious risk factor for suicide	topic_bd
76669	1	355530	7	NULL	NULL	NULL	NULL	bipolar patients	MedicalFinding		 risk factor for		highest			suicide	MentalProcess				NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a recent study of 32,000 bipolar patients' records,[2] the highest risk factor for suicide was being male and having a comorbid anxiety disorder, compared with being young and having a substance-use disorder, which predicted attempts but not necessarily suicide.	topic_bd
76670	2	355530	7	NULL	NULL	0	NULL	statement 1	Process		occur in					comorbid anxiety disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In a recent study of 32,000 bipolar patients' records,[2] the highest risk factor for suicide was being male and having a comorbid anxiety disorder, compared with being young and having a substance-use disorder, which predicted attempts but not necessarily suicide.	topic_bd
76671	3	355530	7	NULL	NULL	0	NULL	statement 1	Process		occur in					substance-use disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In a recent study of 32,000 bipolar patients' records,[2] the highest risk factor for suicide was being male and having a comorbid anxiety disorder, compared with being young and having a substance-use disorder, which predicted attempts but not necessarily suicide.	topic_bd
76672	4	355530	7	NULL	NULL	0	NULL	statement 2	Process		is higher than					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	In a recent study of 32,000 bipolar patients' records,[2] the highest risk factor for suicide was being male and having a comorbid anxiety disorder, compared with being young and having a substance-use disorder, which predicted attempts but not necessarily suicide.	topic_bd
76468	1	355531	7	NULL	NULL	NULL	NULL	Fluoxetine	Chemical		prevents					bipolar type II	MedicalFinding	major depressive episodes in patients with			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fluoxetine appears superior to lithium in preventing recurrence of major depressive episodes in patients with bipolar type II, according to new research.	topic_bd
76469	2	355531	7	NULL	NULL	0	NULL	 lithium	Chemical		prevents					bipolar type II	MedicalFinding	major depressive episodes in patients with			NULL		0	NULL	NULL	NULL	NULL	NULL	Fluoxetine appears superior to lithium in preventing recurrence of major depressive episodes in patients with bipolar type II, according to new research.	topic_bd
76470	3	355531	7	NULL	NULL	0	NULL	statement 1	Process		is superior than					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Fluoxetine appears superior to lithium in preventing recurrence of major depressive episodes in patients with bipolar type II, according to new research.	topic_bd
76471	1	355532	7	NULL	NULL	0	NULL	lithium	Chemical	patients taking	suffer 					relapse	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Patients taking lithium were at risk of suffering a relapse much sooner than those on fluoxetine (Prozac),	topic_bd
76472	2	355532	7	NULL	NULL	NULL	NULL	fluoxetine	Chemical	patients taking	suffer					relapse	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patients taking lithium were at risk of suffering a relapse much sooner than those on fluoxetine (Prozac),	topic_bd
76473	3	355532	7	NULL	NULL	0	NULL	statement 1	Process	relapse of	sooner than					statement 2	Process	relapse of			NULL		0	NULL	NULL	NULL	NULL	NULL	Patients taking lithium were at risk of suffering a relapse much sooner than those on fluoxetine (Prozac),	topic_bd
76474	1	355535	7	NULL	NULL	0	NULL	 alcohol 	Chemical		does not worsen					mood symptoms	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Among people with bipolar disorder who strictly followed their medication plan, drinking alcohol did not appear to worsen their mood symptoms, hint findings of a small study from The Netherlands.	topic_bd
76475	2	355535	7	NULL	NULL	0	NULL	statement 1	Process		occur in					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Among people with bipolar disorder who strictly followed their medication plan, drinking alcohol did not appear to worsen their mood symptoms, hint findings of a small study from The Netherlands.	topic_bd
76477	1	355538	7	NULL	NULL	0	NULL	bipolar spectrum	MedicalFinding		embraces					mania	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	there is ample evidence to support the hypothesis that a wide bipolar spectrum exists in clinical samples...This spectrum embraces mania, hypomania, recurrent brief hypomania, sporadic brief hypomania and cyclothymia.	topic_bd
76478	2	355538	7	NULL	NULL	0	NULL	bipolar spectrum	MedicalFinding		embraces					hypomania	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	there is ample evidence to support the hypothesis that a wide bipolar spectrum exists in clinical samples...This spectrum embraces mania, hypomania, recurrent brief hypomania, sporadic brief hypomania and cyclothymia.	topic_bd
76479	3	355538	7	NULL	NULL	0	NULL	bipolar spectrum	MedicalFinding		embraces					hypomania	MedicalFinding	recurrent brief 			NULL		0	NULL	NULL	NULL	NULL	NULL	there is ample evidence to support the hypothesis that a wide bipolar spectrum exists in clinical samples...This spectrum embraces mania, hypomania, recurrent brief hypomania, sporadic brief hypomania and cyclothymia.	topic_bd
76480	4	355538	7	NULL	NULL	0	NULL	bipolar spectrum	MedicalFinding		embraces					hypomania	MedicalFinding	sporadic brief 			NULL		0	NULL	NULL	NULL	NULL	NULL	there is ample evidence to support the hypothesis that a wide bipolar spectrum exists in clinical samples...This spectrum embraces mania, hypomania, recurrent brief hypomania, sporadic brief hypomania and cyclothymia.	topic_bd
76481	5	355538	7	NULL	NULL	0	NULL	bipolar spectrum	MedicalFinding		embraces					cyclothymia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	there is ample evidence to support the hypothesis that a wide bipolar spectrum exists in clinical samples...This spectrum embraces mania, hypomania, recurrent brief hypomania, sporadic brief hypomania and cyclothymia.	topic_bd
74788	1	355539	5	NULL	NULL	0	NULL	splenectomy	MedicalProcedure		is a type of					surgical procedure	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	There are different types of treatment for patients with hairy cell leukemia. : splenectomy is a surgical procedure to remove the spleen. 	topic_ll
74789	2	355539	5	NULL	NULL	0	NULL	splenectomy	MedicalFinding		removes					spleen	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	There are different types of treatment for patients with hairy cell leukemia. : splenectomy is a surgical procedure to remove the spleen. 	topic_ll
74791	1	355540	5	NULL	NULL	0	NULL	monoclonal antibody therapy	MedicalProcedure		is a type of					targeted therapy	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibody therapy is a type of targeted therapy being studied in the treatment of hairy cell leukemia.	topic_ll
74792	2	355540	5	NULL	NULL	0	NULL	monoclonal antibody therapy	MedicalProcedure		is used to treat		may be			hairy cell leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibody therapy is a type of targeted therapy being studied in the treatment of hairy cell leukemia.	topic_ll
74820	1	355542	5	NULL	NULL	0	NULL	Hairy (leukemia) cells	Cell		is present in					blood	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	The hairy cell leukemia is newly diagnosed and has not been treated except to relieve symptoms such as weight loss and infections. In untreated hairy cell leukemia, some or all of the following conditions occur: * Hairy (leukemia) cells are found in the blood and bone marrow. * The number of red blood cells, white blood cells, or platelets may be lower than normal. * The spleen may be larger than normal. NULL	topic_ll
74821	2	355542	5	NULL	NULL	0	NULL	Hairy (leukemia) cells	Cell		is present in					bone marrow	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	The hairy cell leukemia is newly diagnosed and has not been treated except to relieve symptoms such as weight loss and infections. In untreated hairy cell leukemia, some or all of the following conditions occur: * Hairy (leukemia) cells are found in the blood and bone marrow. * The number of red blood cells, white blood cells, or platelets may be lower than normal. * The spleen may be larger than normal. NULL	topic_ll
74822	3	355542	5	NULL	NULL	0	NULL	treatment	Process		is not available for					hairy cell leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The hairy cell leukemia is newly diagnosed and has not been treated except to relieve symptoms such as weight loss and infections. In untreated hairy cell leukemia, some or all of the following conditions occur: * Hairy (leukemia) cells are found in the blood and bone marrow. * The number of red blood cells, white blood cells, or platelets may be lower than normal. * The spleen may be larger than normal. NULL	topic_ll
74823	4	355542	5	NULL	NULL	0	NULL	hairy cell leukemia	MedicalFinding	treatment	relieves					weight loss	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The hairy cell leukemia is newly diagnosed and has not been treated except to relieve symptoms such as weight loss and infections. In untreated hairy cell leukemia, some or all of the following conditions occur: * Hairy (leukemia) cells are found in the blood and bone marrow. * The number of red blood cells, white blood cells, or platelets may be lower than normal. * The spleen may be larger than normal. NULL	topic_ll
74824	5	355542	5	NULL	NULL	0	NULL	hairy cell leukemia	MedicalFinding	treatment	relieves					infections	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The hairy cell leukemia is newly diagnosed and has not been treated except to relieve symptoms such as weight loss and infections. In untreated hairy cell leukemia, some or all of the following conditions occur: * Hairy (leukemia) cells are found in the blood and bone marrow. * The number of red blood cells, white blood cells, or platelets may be lower than normal. * The spleen may be larger than normal. NULL	topic_ll
74856	1	355543	5	NULL	NULL	0	NULL	Btk	GP		is					Bruton's tyrosine kinase	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	I found another one -- a Btk (Bruton's tyrosine kinase) Inhibitor, PCI-32765, that is currently in Phase I clinical trials in patients with B cell malignancies (specifically Non-Hodgkin's Lymphoma).  Btk is an essential signalling factor needed for the development of  B-cells.  By inhibiting it, the Btk protein production is blocked and B-cells can't develop.	topic_ll
74857	2	355543	5	NULL	NULL	0	NULL	Btk	GP		is a type of					signalling factor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	I found another one -- a Btk (Bruton's tyrosine kinase) Inhibitor, PCI-32765, that is currently in Phase I clinical trials in patients with B cell malignancies (specifically Non-Hodgkin's Lymphoma).  Btk is an essential signalling factor needed for the development of  B-cells.  By inhibiting it, the Btk protein production is blocked and B-cells can't develop.	topic_ll
74858	3	355543	5	NULL	NULL	0	NULL	Btk	GP		is needed for					B-cells	Cell	development of			NULL		0	NULL	NULL	NULL	NULL	NULL	I found another one -- a Btk (Bruton's tyrosine kinase) Inhibitor, PCI-32765, that is currently in Phase I clinical trials in patients with B cell malignancies (specifically Non-Hodgkin's Lymphoma).  Btk is an essential signalling factor needed for the development of  B-cells.  By inhibiting it, the Btk protein production is blocked and B-cells can't develop.	topic_ll
74859	4	355543	5	NULL	NULL	0	NULL	Btk	GP	inhibition of	blocks					Btk protein	GP	production of			NULL		0	NULL	NULL	NULL	NULL	NULL	I found another one -- a Btk (Bruton's tyrosine kinase) Inhibitor, PCI-32765, that is currently in Phase I clinical trials in patients with B cell malignancies (specifically Non-Hodgkin's Lymphoma).  Btk is an essential signalling factor needed for the development of  B-cells.  By inhibiting it, the Btk protein production is blocked and B-cells can't develop.	topic_ll
74860	5	355543	5	NULL	NULL	0	NULL	statement 4	Process		blocks					B-cells	Cell	development of			NULL		0	NULL	NULL	NULL	NULL	NULL	I found another one -- a Btk (Bruton's tyrosine kinase) Inhibitor, PCI-32765, that is currently in Phase I clinical trials in patients with B cell malignancies (specifically Non-Hodgkin's Lymphoma).  Btk is an essential signalling factor needed for the development of  B-cells.  By inhibiting it, the Btk protein production is blocked and B-cells can't develop.	topic_ll
74861	6	355543	5	NULL	NULL	0	NULL	PCI-32765	Chemical		is an inhibitor of					Btk	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	I found another one -- a Btk (Bruton's tyrosine kinase) Inhibitor, PCI-32765, that is currently in Phase I clinical trials in patients with B cell malignancies (specifically Non-Hodgkin's Lymphoma).  Btk is an essential signalling factor needed for the development of  B-cells.  By inhibiting it, the Btk protein production is blocked and B-cells can't develop.	topic_ll
74862	7	355543	5	NULL	NULL	0	NULL	Non-Hodgkin's Lymphoma	MedicalFinding		is a type of					B cell malignancies	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	I found another one -- a Btk (Bruton's tyrosine kinase) Inhibitor, PCI-32765, that is currently in Phase I clinical trials in patients with B cell malignancies (specifically Non-Hodgkin's Lymphoma).  Btk is an essential signalling factor needed for the development of  B-cells.  By inhibiting it, the Btk protein production is blocked and B-cells can't develop.	topic_ll
74863	8	355543	5	NULL	NULL	0	NULL	PCI-32765	Chemical		treats		potentially			Non-Hodgkin's Lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	I found another one -- a Btk (Bruton's tyrosine kinase) Inhibitor, PCI-32765, that is currently in Phase I clinical trials in patients with B cell malignancies (specifically Non-Hodgkin's Lymphoma).  Btk is an essential signalling factor needed for the development of  B-cells.  By inhibiting it, the Btk protein production is blocked and B-cells can't develop.	topic_ll
74864	1	355544	5	NULL	NULL	0	NULL	leukemia cells	Cell		is addicted to					glucose	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Leukemia cells, like most cancers, are addicted to glucose to generate their energy, but new research shows for the first time that these cells also rely on fatty acid metabolism to grow and to evade cell death.	topic_ll
74865	2	355544	5	NULL	NULL	NULL	NULL	glucose	Chemical		generates					energy	AbstractConcept				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Leukemia cells, like most cancers, are addicted to glucose to generate their energy, but new research shows for the first time that these cells also rely on fatty acid metabolism to grow and to evade cell death.	topic_ll
74866	3	355544	5	NULL	NULL	0	NULL	leukemia cells	Cell		rely on					fatty acid	Chemical	metabolism of			NULL		0	NULL	NULL	NULL	NULL	NULL	Leukemia cells, like most cancers, are addicted to glucose to generate their energy, but new research shows for the first time that these cells also rely on fatty acid metabolism to grow and to evade cell death.	topic_ll
74867	4	355544	5	NULL	NULL	0	NULL	statement 3	Process		is required for					growth	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Leukemia cells, like most cancers, are addicted to glucose to generate their energy, but new research shows for the first time that these cells also rely on fatty acid metabolism to grow and to evade cell death.	topic_ll
74868	5	355544	5	NULL	NULL	0	NULL	leukemia cells	Cell		evade					cell death	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Leukemia cells, like most cancers, are addicted to glucose to generate their energy, but new research shows for the first time that these cells also rely on fatty acid metabolism to grow and to evade cell death.	topic_ll
74869	6	355544	5	NULL	NULL	0	NULL	statement 3	Process		is required for					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Leukemia cells, like most cancers, are addicted to glucose to generate their energy, but new research shows for the first time that these cells also rely on fatty acid metabolism to grow and to evade cell death.	topic_ll
74870	1	355545	5	NULL	NULL	0	NULL	fat oxidation	Process		promote		seems to			leukemia cell	Cell	survival of			NULL		0	NULL	NULL	NULL	NULL	NULL	"More importantly, fat oxidation seems to promote leukemia cell survival. Conversely, shutting off fat oxidation makes the cells vulnerable to self-destruction. If these initial results hold up, inhibitors of fat oxidation may become a new way to treat leukemia patients."	topic_ll
74871	3	355545	5	NULL	NULL	0	NULL	fat oxidation	Process	shutting off	leads to					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	"More importantly, fat oxidation seems to promote leukemia cell survival. Conversely, shutting off fat oxidation makes the cells vulnerable to self-destruction. If these initial results hold up, inhibitors of fat oxidation may become a new way to treat leukemia patients."	topic_ll
74872	2	355545	5	NULL	NULL	0	NULL	leukemia cells	Cell		is vulnerable to					self-destruction	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	"More importantly, fat oxidation seems to promote leukemia cell survival. Conversely, shutting off fat oxidation makes the cells vulnerable to self-destruction. If these initial results hold up, inhibitors of fat oxidation may become a new way to treat leukemia patients."	topic_ll
74873	4	355545	5	NULL	NULL	0	NULL	fat oxidation inhibitors	AbstractConcept		treats		potentially			leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	"More importantly, fat oxidation seems to promote leukemia cell survival. Conversely, shutting off fat oxidation makes the cells vulnerable to self-destruction. If these initial results hold up, inhibitors of fat oxidation may become a new way to treat leukemia patients."	topic_ll
74874	1	355546	5	NULL	NULL	0	NULL	etomoxir	Chemical		inhibits					fatty acid	Chemical	oxidation of			NULL		0	NULL	NULL	NULL	NULL	NULL	The team, led by Michael Andreeff and Heinrich Taegtmeyer, found that inhibition of fatty acid oxidation with either etomoxir, a drug that was tested in clinical trials for the treatment of heart disease but never made it to market due to unacceptable toxicities, or ranolazine, a drug approved for the treatment of chronic angina, inhibited human leukemic cell proliferation in vitro.	topic_ll
74884	2	355546	5	NULL	NULL	0	NULL	ranolazine	Chemical		inhibits					fatty acid\t\t	Chemical	oxidation of			NULL		0	NULL	NULL	NULL	NULL	NULL	The team, led by Michael Andreeff and Heinrich Taegtmeyer, found that inhibition of fatty acid oxidation with either etomoxir, a drug that was tested in clinical trials for the treatment of heart disease but never made it to market due to unacceptable toxicities, or ranolazine, a drug approved for the treatment of chronic angina, inhibited human leukemic cell proliferation in vitro.	topic_ll
74885	3	355546	5	NULL	NULL	NULL	NULL	statement 1	Process		inhibits					leukemic cell	Cell	proliferation of;;human			NULL	in vitro	NULL	NULL	NULL	NULL	NULL	NULL	The team, led by Michael Andreeff and Heinrich Taegtmeyer, found that inhibition of fatty acid oxidation with either etomoxir, a drug that was tested in clinical trials for the treatment of heart disease but never made it to market due to unacceptable toxicities, or ranolazine, a drug approved for the treatment of chronic angina, inhibited human leukemic cell proliferation in vitro.	topic_ll
74886	4	355546	5	NULL	NULL	NULL	NULL	statement 2	Process		inhibits					leukemic cell	Cell	proliferation of;;human			NULL	in vitro	NULL	NULL	NULL	NULL	NULL	NULL	The team, led by Michael Andreeff and Heinrich Taegtmeyer, found that inhibition of fatty acid oxidation with either etomoxir, a drug that was tested in clinical trials for the treatment of heart disease but never made it to market due to unacceptable toxicities, or ranolazine, a drug approved for the treatment of chronic angina, inhibited human leukemic cell proliferation in vitro.	topic_ll
74887	5	355546	5	NULL	NULL	0	NULL	ranolazine	Chemical		is a type of					drug	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The team, led by Michael Andreeff and Heinrich Taegtmeyer, found that inhibition of fatty acid oxidation with either etomoxir, a drug that was tested in clinical trials for the treatment of heart disease but never made it to market due to unacceptable toxicities, or ranolazine, a drug approved for the treatment of chronic angina, inhibited human leukemic cell proliferation in vitro.	topic_ll
74888	6	355546	5	NULL	NULL	0	NULL	ranolazine	Chemical		is approved for					chronic angina	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	The team, led by Michael Andreeff and Heinrich Taegtmeyer, found that inhibition of fatty acid oxidation with either etomoxir, a drug that was tested in clinical trials for the treatment of heart disease but never made it to market due to unacceptable toxicities, or ranolazine, a drug approved for the treatment of chronic angina, inhibited human leukemic cell proliferation in vitro.	topic_ll
74889	7	355546	5	NULL	NULL	0	NULL	etomoxir	Chemical		is a type of					drug	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The team, led by Michael Andreeff and Heinrich Taegtmeyer, found that inhibition of fatty acid oxidation with either etomoxir, a drug that was tested in clinical trials for the treatment of heart disease but never made it to market due to unacceptable toxicities, or ranolazine, a drug approved for the treatment of chronic angina, inhibited human leukemic cell proliferation in vitro.	topic_ll
74890	8	355546	5	NULL	NULL	0	NULL	etomoxir	Chemical		is not approved for					heart disease	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	The team, led by Michael Andreeff and Heinrich Taegtmeyer, found that inhibition of fatty acid oxidation with either etomoxir, a drug that was tested in clinical trials for the treatment of heart disease but never made it to market due to unacceptable toxicities, or ranolazine, a drug approved for the treatment of chronic angina, inhibited human leukemic cell proliferation in vitro.	topic_ll
74891	9	355546	5	NULL	NULL	0	NULL	toxicities	AbstractConcept	unacceptable	leads to					statement 8	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The team, led by Michael Andreeff and Heinrich Taegtmeyer, found that inhibition of fatty acid oxidation with either etomoxir, a drug that was tested in clinical trials for the treatment of heart disease but never made it to market due to unacceptable toxicities, or ranolazine, a drug approved for the treatment of chronic angina, inhibited human leukemic cell proliferation in vitro.	topic_ll
74892	1	355548	5	NULL	NULL	0	NULL	Gfi1b	GP		is inactivated in					stem cells	Cell	transplanted			NULL		0	NULL	NULL	NULL	NULL	NULL	inactivation of Gfi1b in the transplanted stem cells could accelerate the production of new blood cells, thus making stem cell therapy more efficient and less dangerous for the patient.	topic_ll
74893	2	355548	5	NULL	NULL	0	NULL	statement 1	Process		accelerates					blood cells	Cell	production of;;new			NULL		0	NULL	NULL	NULL	NULL	NULL	inactivation of Gfi1b in the transplanted stem cells could accelerate the production of new blood cells, thus making stem cell therapy more efficient and less dangerous for the patient.	topic_ll
74894	3	355548	5	NULL	NULL	0	NULL	stem cell therapy	MedicalProcedure		is more efficient for					patient	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	inactivation of Gfi1b in the transplanted stem cells could accelerate the production of new blood cells, thus making stem cell therapy more efficient and less dangerous for the patient.	topic_ll
74895	4	355548	5	NULL	NULL	0	NULL	stem cell therapy	MedicalProcedure		is less dangerous for					patient	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	inactivation of Gfi1b in the transplanted stem cells could accelerate the production of new blood cells, thus making stem cell therapy more efficient and less dangerous for the patient.	topic_ll
74896	1	355549	5	NULL	NULL	0	NULL	AHI-1 protein	GP		is present in					leukemia cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	The team found that a protein called AHI-1, which has been found in leukemia cells in the past, is highly expressed in CML stem cells.	topic_ll
74897	2	355549	5	NULL	NULL	0	NULL	AHI-1 protein	GP		is expressed in		highly			CML stem cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	The team found that a protein called AHI-1, which has been found in leukemia cells in the past, is highly expressed in CML stem cells.	topic_ll
74898	1	355551	5	NULL	NULL	0	NULL	RRLON	MedicalFinding		is a side-effect of					Rituxan	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	but after some more investigation, my best guess is that I've experienced a side-effect of Rituxan known as Rituxan related late onset  neutropenia  (RRLON).  	topic_ll
74899	2	355551	5	NULL	NULL	0	NULL	RRLON	MedicalFinding		is					Rituxan related late onset neutropenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	but after some more investigation, my best guess is that I've experienced a side-effect of Rituxan known as Rituxan related late onset  neutropenia  (RRLON).  	topic_ll
74900	1	355552	5	NULL	NULL	0	NULL	HCL	MedicalFinding		is a disorder of		uncommon;;chronic;;neoplastic 			B lymphocytes	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	HCL is an uncommon, chronic, neoplastic (malignant) disorder of B lymphocytes (a type of white blood cell) that afflicts middle-aged men. The patient usually presents with pancytopenia (broad spectrum reduction in blood counts -- low platelets, low white blood cells, low red blood cells).	topic_ll
74901	2	355552	5	NULL	NULL	0	NULL	B lymphocytes	Cell		is a type of					white blood cell	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	HCL is an uncommon, chronic, neoplastic (malignant) disorder of B lymphocytes (a type of white blood cell) that afflicts middle-aged men. The patient usually presents with pancytopenia (broad spectrum reduction in blood counts -- low platelets, low white blood cells, low red blood cells).	topic_ll
74902	3	355552	5	NULL	NULL	NULL	NULL	HCL	MedicalFinding		afflicts					men	GroupOfPeople	middle-aged			NULL		NULL	NULL	NULL	NULL	NULL	NULL	HCL is an uncommon, chronic, neoplastic (malignant) disorder of B lymphocytes (a type of white blood cell) that afflicts middle-aged men. The patient usually presents with pancytopenia (broad spectrum reduction in blood counts -- low platelets, low white blood cells, low red blood cells).	topic_ll
74903	4	355552	5	NULL	NULL	0	NULL	HCL patients	GroupOfPeople		presents with					pancytopenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	HCL is an uncommon, chronic, neoplastic (malignant) disorder of B lymphocytes (a type of white blood cell) that afflicts middle-aged men. The patient usually presents with pancytopenia (broad spectrum reduction in blood counts -- low platelets, low white blood cells, low red blood cells).	topic_ll
74904	5	355552	5	NULL	NULL	0	NULL	blood counts	AbstractConcept	reduction of	is known as					pancytopenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	HCL is an uncommon, chronic, neoplastic (malignant) disorder of B lymphocytes (a type of white blood cell) that afflicts middle-aged men. The patient usually presents with pancytopenia (broad spectrum reduction in blood counts -- low platelets, low white blood cells, low red blood cells).	topic_ll
74905	6	355552	5	NULL	NULL	0	NULL	platelets	Cell		is a type of					blood cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	HCL is an uncommon, chronic, neoplastic (malignant) disorder of B lymphocytes (a type of white blood cell) that afflicts middle-aged men. The patient usually presents with pancytopenia (broad spectrum reduction in blood counts -- low platelets, low white blood cells, low red blood cells).	topic_ll
74906	7	355552	5	NULL	NULL	0	NULL	white blood cells	Cell		is a type of					blood cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	HCL is an uncommon, chronic, neoplastic (malignant) disorder of B lymphocytes (a type of white blood cell) that afflicts middle-aged men. The patient usually presents with pancytopenia (broad spectrum reduction in blood counts -- low platelets, low white blood cells, low red blood cells).	topic_ll
74907	8	355552	5	NULL	NULL	0	NULL	 red blood cells	Cell		is a type of					blood cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	HCL is an uncommon, chronic, neoplastic (malignant) disorder of B lymphocytes (a type of white blood cell) that afflicts middle-aged men. The patient usually presents with pancytopenia (broad spectrum reduction in blood counts -- low platelets, low white blood cells, low red blood cells).	topic_ll
74908	1	355554	5	NULL	NULL	0	NULL	caffeine	Chemical		lowers					TNFa	GP	levels of			NULL		0	NULL	NULL	NULL	NULL	NULL	After my testing in August, I blogged about some research which indicated that caffeine can lower TNFa levels and hypothesized that since some research indicates that HCL apparently thrives on TNFa, maybe drinking coffee and consuming other TNFa lowering foods may improve or sustain my response.	topic_ll
74909	2	355554	5	NULL	NULL	0	NULL	HCL	MedicalFinding		thrives on		apparently			TNFa	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	After my testing in August, I blogged about some research which indicated that caffeine can lower TNFa levels and hypothesized that since some research indicates that HCL apparently thrives on TNFa, maybe drinking coffee and consuming other TNFa lowering foods may improve or sustain my response.	topic_ll
74910	1	355555	5	NULL	NULL	0	NULL	HCL	MedicalFinding	risk of	is concentrated in					males	GroupOfPeople	white			NULL		0	NULL	NULL	NULL	NULL	NULL	HCL risk was concentrated in white males; there were few black and Asian patients for analysis.	topic_ll
74911	1	355556	5	NULL	NULL	0	NULL	HCL	MedicalFinding	risk of	is concentrated in					males	GroupOfPeople	white			NULL		0	NULL	NULL	NULL	NULL	NULL	HCL risk was concentrated in white males; there were few black and Asian patients for analysis. Using data from all cancer patients diagnosed during the study period, Jewish men had significantly greater risk of HCL than Protestant men.	topic_ll
74912	2	355556	5	NULL	NULL	0	NULL	men	GroupOfPeople	Jewish	is at risk of					HCL	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	HCL risk was concentrated in white males; there were few black and Asian patients for analysis. Using data from all cancer patients diagnosed during the study period, Jewish men had significantly greater risk of HCL than Protestant men.	topic_ll
74913	3	355556	5	NULL	NULL	0	NULL	men	GroupOfPeople	Protestant	is at risk of					HCL	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	HCL risk was concentrated in white males; there were few black and Asian patients for analysis. Using data from all cancer patients diagnosed during the study period, Jewish men had significantly greater risk of HCL than Protestant men.	topic_ll
74914	4	355556	5	NULL	NULL	0	NULL	statement 2	Process		greater than		significantly			statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	HCL risk was concentrated in white males; there were few black and Asian patients for analysis. Using data from all cancer patients diagnosed during the study period, Jewish men had significantly greater risk of HCL than Protestant men.	topic_ll
74915	1	355558	5	NULL	NULL	0	NULL	GSE	CellComponent		is					grape seed extract	CellComponent				NULL		0	NULL	NULL	NULL	NULL	NULL	cell death effects of Grape Seed Extract (GSE) on Jurkat cells through increased activation of JNK enzymes in these leukemic T-cells. Prior studies of GSE in Jurkat cells as well as prostate cancer show that GSE is highly effective in activating JNK enzymes and inducing apoptosis in those cell lines.	topic_ll
74916	2	355558	5	NULL	NULL	NULL	NULL	GSE	CellComponent		activates		effectively			JNK enzymes	GP				NULL	Jurkat cells	NULL	NULL	NULL	NULL	NULL	NULL	cell death effects of Grape Seed Extract (GSE) on Jurkat cells through increased activation of JNK enzymes in these leukemic T-cells. Prior studies of GSE in Jurkat cells as well as prostate cancer show that GSE is highly effective in activating JNK enzymes and inducing apoptosis in those cell lines.	topic_ll
74917	3	355558	5	NULL	NULL	NULL	NULL	statement 2	Process		induce					apoptosis	Process				NULL	Jurkat cells	NULL	NULL	NULL	NULL	NULL	NULL	cell death effects of Grape Seed Extract (GSE) on Jurkat cells through increased activation of JNK enzymes in these leukemic T-cells. Prior studies of GSE in Jurkat cells as well as prostate cancer show that GSE is highly effective in activating JNK enzymes and inducing apoptosis in those cell lines.	topic_ll
74922	4	355558	5	NULL	NULL	NULL	NULL	GSE	CellComponent		activates		effectively			JNK enzymes	GP				NULL	prostate cancer	NULL	NULL	NULL	NULL	NULL	NULL	cell death effects of Grape Seed Extract (GSE) on Jurkat cells through increased activation of JNK enzymes in these leukemic T-cells. Prior studies of GSE in Jurkat cells as well as prostate cancer show that GSE is highly effective in activating JNK enzymes and inducing apoptosis in those cell lines.	topic_ll
74923	5	355558	5	NULL	NULL	0	NULL	statement 4	Process		induce					apoptosis	Process				NULL	prostate cancer	0	NULL	NULL	NULL	NULL	NULL	cell death effects of Grape Seed Extract (GSE) on Jurkat cells through increased activation of JNK enzymes in these leukemic T-cells. Prior studies of GSE in Jurkat cells as well as prostate cancer show that GSE is highly effective in activating JNK enzymes and inducing apoptosis in those cell lines.	topic_ll
74966	6	355558	5	NULL	NULL	NULL	NULL	GSE	CellComponent		effects					cell death	Process				NULL	Jurkat cells	NULL	NULL	NULL	NULL	NULL	NULL	cell death effects of Grape Seed Extract (GSE) on Jurkat cells through increased activation of JNK enzymes in these leukemic T-cells. Prior studies of GSE in Jurkat cells as well as prostate cancer show that GSE is highly effective in activating JNK enzymes and inducing apoptosis in those cell lines.	topic_ll
74967	7	355558	5	NULL	NULL	0	NULL	statement 6	Process		occurs through					JNK enzymes	GP	increased activation of			NULL	leukemic T-cells	0	NULL	NULL	NULL	NULL	NULL	cell death effects of Grape Seed Extract (GSE) on Jurkat cells through increased activation of JNK enzymes in these leukemic T-cells. Prior studies of GSE in Jurkat cells as well as prostate cancer show that GSE is highly effective in activating JNK enzymes and inducing apoptosis in those cell lines.	topic_ll
74918	1	355559	5	NULL	NULL	NULL	NULL	GSE	CellComponent		activates		effectively			JNK enzymes	GP				NULL	Jurkat cells	NULL	NULL	NULL	NULL	NULL	NULL	Prior studies of GSE in Jurkat cells as well as prostate cancer show that GSE is highly effective in activating JNK enzymes and inducing apoptosis in those cell lines. 	topic_ll
74919	2	355559	5	NULL	NULL	0	NULL	GSE	CellComponent		activates		effectively			JNK enzymes	GP				NULL	prostate cancer	0	NULL	NULL	NULL	NULL	NULL	Prior studies of GSE in Jurkat cells as well as prostate cancer show that GSE is highly effective in activating JNK enzymes and inducing apoptosis in those cell lines. 	topic_ll
74920	3	355559	5	NULL	NULL	0	NULL	statement 1	Process		induce					apoptosis	Process				NULL	Jurkat cells	0	NULL	NULL	NULL	NULL	NULL	Prior studies of GSE in Jurkat cells as well as prostate cancer show that GSE is highly effective in activating JNK enzymes and inducing apoptosis in those cell lines. 	topic_ll
74921	4	355559	5	NULL	NULL	NULL	NULL	statement 2	Process		induce					apoptosis	Process				NULL	prostate cancer	NULL	NULL	NULL	NULL	NULL	NULL	Prior studies of GSE in Jurkat cells as well as prostate cancer show that GSE is highly effective in activating JNK enzymes and inducing apoptosis in those cell lines. 	topic_ll
74968	1	355561	5	NULL	NULL	0	NULL	Aloe-Emodin	Chemical		is present in					Rhubarb	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Aloe-Emodin, found in Rhubarb and Aloe, is also a pronounced JNK activator and apoptosis agent. Rhubarb is also a known blood thinner which could cause spontaneous bleeding in individuals with Thrombocytopenia or clinical HCL.	topic_ll
74969	2	355561	5	NULL	NULL	0	NULL	Aloe-Emodin	Chemical		is present in					Aloe	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Aloe-Emodin, found in Rhubarb and Aloe, is also a pronounced JNK activator and apoptosis agent. Rhubarb is also a known blood thinner which could cause spontaneous bleeding in individuals with Thrombocytopenia or clinical HCL.	topic_ll
74970	3	355561	5	NULL	NULL	0	NULL	Aloe-Emodin	Chemical		is an activator of		pronounced			JNK	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Aloe-Emodin, found in Rhubarb and Aloe, is also a pronounced JNK activator and apoptosis agent. Rhubarb is also a known blood thinner which could cause spontaneous bleeding in individuals with Thrombocytopenia or clinical HCL.	topic_ll
74971	4	355561	5	NULL	NULL	0	NULL	Aloe-Emodin	Chemical		is a type of					apoptosis agent	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Aloe-Emodin, found in Rhubarb and Aloe, is also a pronounced JNK activator and apoptosis agent. Rhubarb is also a known blood thinner which could cause spontaneous bleeding in individuals with Thrombocytopenia or clinical HCL.	topic_ll
74972	5	355561	5	NULL	NULL	0	NULL	Rhubarb	Chemical		is a type of					blood thinner	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Aloe-Emodin, found in Rhubarb and Aloe, is also a pronounced JNK activator and apoptosis agent. Rhubarb is also a known blood thinner which could cause spontaneous bleeding in individuals with Thrombocytopenia or clinical HCL.	topic_ll
74973	6	355561	5	NULL	NULL	0	NULL	Rhubarb	Chemical		cause					spontaneous bleeding	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Aloe-Emodin, found in Rhubarb and Aloe, is also a pronounced JNK activator and apoptosis agent. Rhubarb is also a known blood thinner which could cause spontaneous bleeding in individuals with Thrombocytopenia or clinical HCL.	topic_ll
74974	7	355561	5	NULL	NULL	0	NULL	statement 6	Process		occurs in					Thrombocytopenia individuals	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Aloe-Emodin, found in Rhubarb and Aloe, is also a pronounced JNK activator and apoptosis agent. Rhubarb is also a known blood thinner which could cause spontaneous bleeding in individuals with Thrombocytopenia or clinical HCL.	topic_ll
74975	8	355561	5	NULL	NULL	0	NULL	statement 6	Process		occurs in					clinical HCL individuals	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Aloe-Emodin, found in Rhubarb and Aloe, is also a pronounced JNK activator and apoptosis agent. Rhubarb is also a known blood thinner which could cause spontaneous bleeding in individuals with Thrombocytopenia or clinical HCL.	topic_ll
74976	1	355562	5	NULL	NULL	0	NULL	decoy IL-1 receptor	GP		is present in					hairy cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	This same research indicates that hairy cells may have a decoy IL-1 (interleukin) receptor 	topic_ll
74977	2	355562	5	NULL	NULL	0	NULL	IL	GP		is					interleukin	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	This same research indicates that hairy cells may have a decoy IL-1 (interleukin) receptor 	topic_ll
74978	1	355563	5	NULL	NULL	0	NULL	hairy cell leukemia	MedicalFinding		consumes					cholesterol	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	hairy cell leukemia also consumes cholesterol. Several studies have shown that hairy cells contain more cholesterol than their normal B-cell counterparts. Likewise, patients with hairy cell leukemia typically have low levels of both LDL (bad) and HDL (good) cholesterol.	topic_ll
74979	2	355563	5	NULL	NULL	0	NULL	hairy cells	Cell		contains					cholesterol	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	hairy cell leukemia also consumes cholesterol. Several studies have shown that hairy cells contain more cholesterol than their normal B-cell counterparts. Likewise, patients with hairy cell leukemia typically have low levels of both LDL (bad) and HDL (good) cholesterol.	topic_ll
74980	3	355563	5	NULL	NULL	0	NULL	B-cell counterparts	Cell	normal	contains					cholesterol	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	hairy cell leukemia also consumes cholesterol. Several studies have shown that hairy cells contain more cholesterol than their normal B-cell counterparts. Likewise, patients with hairy cell leukemia typically have low levels of both LDL (bad) and HDL (good) cholesterol.	topic_ll
74981	4	355563	5	NULL	NULL	0	NULL	statement 2	Process		is more than					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	hairy cell leukemia also consumes cholesterol. Several studies have shown that hairy cells contain more cholesterol than their normal B-cell counterparts. Likewise, patients with hairy cell leukemia typically have low levels of both LDL (bad) and HDL (good) cholesterol.	topic_ll
74982	5	355563	5	NULL	NULL	0	NULL	LDL Cholestrol	Chemical	level of	is low in					hairy cell leukemia pateints	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	hairy cell leukemia also consumes cholesterol. Several studies have shown that hairy cells contain more cholesterol than their normal B-cell counterparts. Likewise, patients with hairy cell leukemia typically have low levels of both LDL (bad) and HDL (good) cholesterol.	topic_ll
74983	6	355563	5	NULL	NULL	0	NULL	HDL Cholestrol	Chemical	level of	is low in					hairy cell leukemia pateints	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	hairy cell leukemia also consumes cholesterol. Several studies have shown that hairy cells contain more cholesterol than their normal B-cell counterparts. Likewise, patients with hairy cell leukemia typically have low levels of both LDL (bad) and HDL (good) cholesterol.	topic_ll
74997	1	355564	5	NULL	NULL	0	NULL	LDL cholesterol	Chemical	level of	is low in					 hairy cell leukemia patients	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise, patients with hairy cell leukemia typically have low levels of both LDL (bad) and HDL (good) cholesterol.	topic_ll
74998	2	355564	5	NULL	NULL	0	NULL	HDL cholesterol	Chemical	level of	is low in					hairy cell leukemia patients	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise, patients with hairy cell leukemia typically have low levels of both LDL (bad) and HDL (good) cholesterol.	topic_ll
75002	1	355565	5	NULL	NULL	0	NULL	Theory of Mind deficit	MedicalFinding		is observed in					autistic individuals	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	It is now widely accepted that individuals with autism have a Theory of Mind (ToM) or mentalizing deficit	topic_aut
75003	2	355565	5	NULL	NULL	0	NULL	Theory of Mind	MentalProcess		is also known as					mentalizing	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	It is now widely accepted that individuals with autism have a Theory of Mind (ToM) or mentalizing deficit	topic_aut
76482	1	355580	7	NULL	NULL	0	NULL	migraine	MedicalFinding		associated with					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	There would also be a trend towards an association of migraine with bipolar disorder, but not with substance abuse/dependence.	topic_bd
76483	2	355580	7	NULL	NULL	0	NULL	migraine	MedicalFinding		not associated with					substance abuse/dependence	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	There would also be a trend towards an association of migraine with bipolar disorder, but not with substance abuse/dependence.	topic_bd
75004	1	355589	5	NULL	NULL	0	NULL	PBSCs	Cell		is					peripheral blood stem cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	These multipotent peripheral blood stem cells, or PBSCs, can be used just like bone marrow stem cells to treat leukemia, other cancers and various blood disorders. 	topic_ll
75005	2	355589	5	NULL	NULL	0	NULL	bone marrow stem cells	Cell		is used to treat					leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	These multipotent peripheral blood stem cells, or PBSCs, can be used just like bone marrow stem cells to treat leukemia, other cancers and various blood disorders. 	topic_ll
75006	3	355589	5	NULL	NULL	0	NULL	PBSCs	Cell	multipotent 	is used to treat					leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	These multipotent peripheral blood stem cells, or PBSCs, can be used just like bone marrow stem cells to treat leukemia, other cancers and various blood disorders. 	topic_ll
75007	4	355589	5	NULL	NULL	NULL	NULL	PBSCs	Cell	multipotent	is used to treat					cancer	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	These multipotent peripheral blood stem cells, or PBSCs, can be used just like bone marrow stem cells to treat leukemia, other cancers and various blood disorders. 	topic_ll
75008	5	355589	5	NULL	NULL	0	NULL	PBSCs	Cell	multipotent	is used to treat					 blood disorders	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	These multipotent peripheral blood stem cells, or PBSCs, can be used just like bone marrow stem cells to treat leukemia, other cancers and various blood disorders. 	topic_ll
75009	1	355590	5	NULL	NULL	0	NULL	stem-cell-rich blood	OrganismPart	multipotent	is present in					umbilical cord	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	the multipotent-stem-cell-rich blood found in the umbilical cord has proven useful in treating the same types of health problems as those treated using bone marrow stem cells and PBSCs. Umbilical cord blood stem cell transplants are less prone to rejection than either bone marrow or peripheral blood stem cells.	topic_ll
75014	2	355590	5	NULL	NULL	NULL	NULL	stem cell transplants	Cell	umbilical cord blood 	is prone to					rejection	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	the multipotent-stem-cell-rich blood found in the umbilical cord has proven useful in treating the same types of health problems as those treated using bone marrow stem cells and PBSCs. Umbilical cord blood stem cell transplants are less prone to rejection than either bone marrow or peripheral blood stem cells.	topic_ll
75015	3	355590	5	NULL	NULL	0	NULL	bone marrow	OrganismPart		is prone to					rejection	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	the multipotent-stem-cell-rich blood found in the umbilical cord has proven useful in treating the same types of health problems as those treated using bone marrow stem cells and PBSCs. Umbilical cord blood stem cell transplants are less prone to rejection than either bone marrow or peripheral blood stem cells.	topic_ll
75016	4	355590	5	NULL	NULL	0	NULL	peripheral blood stem cells	Cell		is prone to					rejection	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	the multipotent-stem-cell-rich blood found in the umbilical cord has proven useful in treating the same types of health problems as those treated using bone marrow stem cells and PBSCs. Umbilical cord blood stem cell transplants are less prone to rejection than either bone marrow or peripheral blood stem cells.	topic_ll
75017	5	355590	5	NULL	NULL	0	NULL	statement 2	Process		lesser than					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	the multipotent-stem-cell-rich blood found in the umbilical cord has proven useful in treating the same types of health problems as those treated using bone marrow stem cells and PBSCs. Umbilical cord blood stem cell transplants are less prone to rejection than either bone marrow or peripheral blood stem cells.	topic_ll
75018	6	355590	5	NULL	NULL	0	NULL	statement 2	Process		lesser than					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	the multipotent-stem-cell-rich blood found in the umbilical cord has proven useful in treating the same types of health problems as those treated using bone marrow stem cells and PBSCs. Umbilical cord blood stem cell transplants are less prone to rejection than either bone marrow or peripheral blood stem cells.	topic_ll
75023	1	355591	5	NULL	NULL	0	NULL	HyperCVAD	Chemical		is a type of					chemotherapy regimen	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	HyperCVAD is a chemotherapy regimen used to treat some forms of leukemia, non-Hodgkin lymphoma (high grade) and lymphoblastic lymphoma.	topic_ll
75024	2	355591	5	NULL	NULL	0	NULL	HyperCVAD	Chemical		is used to treat					leukemia	MedicalFinding	some forms of			NULL		0	NULL	NULL	NULL	NULL	NULL	HyperCVAD is a chemotherapy regimen used to treat some forms of leukemia, non-Hodgkin lymphoma (high grade) and lymphoblastic lymphoma.	topic_ll
75025	3	355591	5	NULL	NULL	0	NULL	HyperCVAD	Chemical		is used to treat					non-Hodgkin lymphoma (high grade)	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	HyperCVAD is a chemotherapy regimen used to treat some forms of leukemia, non-Hodgkin lymphoma (high grade) and lymphoblastic lymphoma.	topic_ll
75026	4	355591	5	NULL	NULL	0	NULL	HyperCVAD	Chemical		is used to treat					lymphoblastic lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	HyperCVAD is a chemotherapy regimen used to treat some forms of leukemia, non-Hodgkin lymphoma (high grade) and lymphoblastic lymphoma.	topic_ll
75029	1	355593	5	NULL	NULL	NULL	NULL	vegetables	Organism	consumption of	reduce					leukemia	MedicalFinding	risk of;;adult			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diet and Adult Leukemia Risk: The findings of this study indicate that people eating at least three to four servings of vegetables per day appear to have 44% lower risk when compared to people eating less vegetables. 	topic_ll
75031	1	355594	5	NULL	NULL	0	NULL	fruit	OrganismPart		rich in					vitamin C	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Overall, the study results suggest that during the first two years of life, regular consumption of fruits and fruit juices high in vitamin C and or potassium may reduce the risk of childhood leukemia	topic_ll
75033	2	355594	5	NULL	NULL	0	NULL	fruit juice	AbstractConcept		rich in					vitamin C	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Overall, the study results suggest that during the first two years of life, regular consumption of fruits and fruit juices high in vitamin C and or potassium may reduce the risk of childhood leukemia	topic_ll
75034	3	355594	5	NULL	NULL	0	NULL	fruit	OrganismPart		rich in					potassium	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Overall, the study results suggest that during the first two years of life, regular consumption of fruits and fruit juices high in vitamin C and or potassium may reduce the risk of childhood leukemia	topic_ll
75035	4	355594	5	NULL	NULL	0	NULL	fruit juice	AbstractConcept		rich in					potassium	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Overall, the study results suggest that during the first two years of life, regular consumption of fruits and fruit juices high in vitamin C and or potassium may reduce the risk of childhood leukemia	topic_ll
75037	5	355594	5	NULL	NULL	0	NULL	statement 1	Process	regular consumption of	reduce					leukemia	MedicalFinding	risk of;;childhood			NULL		0	NULL	NULL	NULL	NULL	NULL	Overall, the study results suggest that during the first two years of life, regular consumption of fruits and fruit juices high in vitamin C and or potassium may reduce the risk of childhood leukemia	topic_ll
75038	6	355594	5	NULL	NULL	0	NULL	statement 2	Process	regular consumption of	reduce					leukemia	MedicalFinding	risk of;;childhood			NULL		0	NULL	NULL	NULL	NULL	NULL	Overall, the study results suggest that during the first two years of life, regular consumption of fruits and fruit juices high in vitamin C and or potassium may reduce the risk of childhood leukemia	topic_ll
75040	7	355594	5	NULL	NULL	0	NULL	statement 3	Process	regular consumption of	reduce					leukemia	MedicalFinding	risk of;;childhood			NULL		0	NULL	NULL	NULL	NULL	NULL	Overall, the study results suggest that during the first two years of life, regular consumption of fruits and fruit juices high in vitamin C and or potassium may reduce the risk of childhood leukemia	topic_ll
75042	8	355594	5	NULL	NULL	0	NULL	statement 4	Process	regular consumption of	reduce					leukemia	MedicalFinding	risk of;;childhood			NULL		0	NULL	NULL	NULL	NULL	NULL	Overall, the study results suggest that during the first two years of life, regular consumption of fruits and fruit juices high in vitamin C and or potassium may reduce the risk of childhood leukemia	topic_ll
75043	1	355595	5	NULL	NULL	0	NULL	bioflavonoids	Chemical		breaks					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	Scientists from the University of Chicago Medical Center have found molecular evidence that bioflavonoids, which are ordinarily considered quite beneficial, can cause breaks in DNA that could trigger the development of infant leukemias.	topic_ll
75044	2	355595	5	NULL	NULL	0	NULL	statement 1	Process		triggers					leukemia	MedicalFinding	development of;;infant			NULL		0	NULL	NULL	NULL	NULL	NULL	Scientists from the University of Chicago Medical Center have found molecular evidence that bioflavonoids, which are ordinarily considered quite beneficial, can cause breaks in DNA that could trigger the development of infant leukemias.	topic_ll
75045	1	355596	5	NULL	NULL	0	NULL	bioflavonoids	Chemical		breaks					DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	Scientists from the University of Chicago Medical Center have found molecular evidence that bioflavonoids, which are ordinarily considered quite beneficial, can cause breaks in DNA that could trigger the development of infant leukemias. Certain types of bioflavonoids, especially the flavonols, were more powerful topo-II inhibitors than others. For example, two different forms of quercetin, a dietary supplement, and fisetin, which is derived from herbs, were equal to VP16 in triggering MLL cleavage. 	topic_ll
75046	2	355596	5	NULL	NULL	0	NULL	statement 1	Process		triggers					leukemia	MedicalFinding	development of;;infant			NULL		0	NULL	NULL	NULL	NULL	NULL	Scientists from the University of Chicago Medical Center have found molecular evidence that bioflavonoids, which are ordinarily considered quite beneficial, can cause breaks in DNA that could trigger the development of infant leukemias. Certain types of bioflavonoids, especially the flavonols, were more powerful topo-II inhibitors than others. For example, two different forms of quercetin, a dietary supplement, and fisetin, which is derived from herbs, were equal to VP16 in triggering MLL cleavage. 	topic_ll
75047	3	355596	5	NULL	NULL	0	NULL	flavonols	Chemical		is a type of					bioflavonoids	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Scientists from the University of Chicago Medical Center have found molecular evidence that bioflavonoids, which are ordinarily considered quite beneficial, can cause breaks in DNA that could trigger the development of infant leukemias. Certain types of bioflavonoids, especially the flavonols, were more powerful topo-II inhibitors than others. For example, two different forms of quercetin, a dietary supplement, and fisetin, which is derived from herbs, were equal to VP16 in triggering MLL cleavage. 	topic_ll
75048	4	355596	5	NULL	NULL	0	NULL	flavonols	Chemical		is an inhibitor of		powerful			topo-II	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Scientists from the University of Chicago Medical Center have found molecular evidence that bioflavonoids, which are ordinarily considered quite beneficial, can cause breaks in DNA that could trigger the development of infant leukemias. Certain types of bioflavonoids, especially the flavonols, were more powerful topo-II inhibitors than others. For example, two different forms of quercetin, a dietary supplement, and fisetin, which is derived from herbs, were equal to VP16 in triggering MLL cleavage. 	topic_ll
75049	5	355596	5	NULL	NULL	0	NULL	VP16	Chemical		triggers					MLL	GP	cleavage of			NULL		0	NULL	NULL	NULL	NULL	NULL	Scientists from the University of Chicago Medical Center have found molecular evidence that bioflavonoids, which are ordinarily considered quite beneficial, can cause breaks in DNA that could trigger the development of infant leukemias. Certain types of bioflavonoids, especially the flavonols, were more powerful topo-II inhibitors than others. For example, two different forms of quercetin, a dietary supplement, and fisetin, which is derived from herbs, were equal to VP16 in triggering MLL cleavage. 	topic_ll
75050	6	355596	5	NULL	NULL	0	NULL	quercetin	Chemical		is a type of					dietary supplement	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Scientists from the University of Chicago Medical Center have found molecular evidence that bioflavonoids, which are ordinarily considered quite beneficial, can cause breaks in DNA that could trigger the development of infant leukemias. Certain types of bioflavonoids, especially the flavonols, were more powerful topo-II inhibitors than others. For example, two different forms of quercetin, a dietary supplement, and fisetin, which is derived from herbs, were equal to VP16 in triggering MLL cleavage. 	topic_ll
75177	7	355596	5	NULL	NULL	0	NULL	fisetin	Chemical		is derived from					herbs	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Scientists from the University of Chicago Medical Center have found molecular evidence that bioflavonoids, which are ordinarily considered quite beneficial, can cause breaks in DNA that could trigger the development of infant leukemias. Certain types of bioflavonoids, especially the flavonols, were more powerful topo-II inhibitors than others. For example, two different forms of quercetin, a dietary supplement, and fisetin, which is derived from herbs, were equal to VP16 in triggering MLL cleavage. 	topic_ll
75178	8	355596	5	NULL	NULL	0	NULL	fisetin	Chemical		trigger					MLL	GP	cleavage of			NULL		0	NULL	NULL	NULL	NULL	NULL	Scientists from the University of Chicago Medical Center have found molecular evidence that bioflavonoids, which are ordinarily considered quite beneficial, can cause breaks in DNA that could trigger the development of infant leukemias. Certain types of bioflavonoids, especially the flavonols, were more powerful topo-II inhibitors than others. For example, two different forms of quercetin, a dietary supplement, and fisetin, which is derived from herbs, were equal to VP16 in triggering MLL cleavage. 	topic_ll
75179	9	355596	5	NULL	NULL	0	NULL	quercetin	Chemical		trigger					MLL	GP	cleavage of			NULL		0	NULL	NULL	NULL	NULL	NULL	Scientists from the University of Chicago Medical Center have found molecular evidence that bioflavonoids, which are ordinarily considered quite beneficial, can cause breaks in DNA that could trigger the development of infant leukemias. Certain types of bioflavonoids, especially the flavonols, were more powerful topo-II inhibitors than others. For example, two different forms of quercetin, a dietary supplement, and fisetin, which is derived from herbs, were equal to VP16 in triggering MLL cleavage. 	topic_ll
75180	10	355596	5	NULL	NULL	0	NULL	statement 8	Process		is equal to					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Scientists from the University of Chicago Medical Center have found molecular evidence that bioflavonoids, which are ordinarily considered quite beneficial, can cause breaks in DNA that could trigger the development of infant leukemias. Certain types of bioflavonoids, especially the flavonols, were more powerful topo-II inhibitors than others. For example, two different forms of quercetin, a dietary supplement, and fisetin, which is derived from herbs, were equal to VP16 in triggering MLL cleavage. 	topic_ll
75181	11	355596	5	NULL	NULL	0	NULL	statement 9	Process		is equal to					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Scientists from the University of Chicago Medical Center have found molecular evidence that bioflavonoids, which are ordinarily considered quite beneficial, can cause breaks in DNA that could trigger the development of infant leukemias. Certain types of bioflavonoids, especially the flavonols, were more powerful topo-II inhibitors than others. For example, two different forms of quercetin, a dietary supplement, and fisetin, which is derived from herbs, were equal to VP16 in triggering MLL cleavage. 	topic_ll
75182	1	355599	5	NULL	NULL	0	NULL	MLL	GP		is a type of					promiscuous gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	MLL is a promiscuous gene. Once broken, it can reconnect with any of more than 40 other genes in a translocation, a process that involves an exchange of DNA between two chromosomes. Extensive recombinations usually cause cell death; but subtle translocations involving MLL can result in the rapid, uncontrolled cell division seen in leukemia.	topic_ll
75183	2	355599	5	NULL	NULL	0	NULL	MLL gene	GP	broken	reconnect with					gene	GP	any			NULL		0	NULL	NULL	NULL	NULL	NULL	MLL is a promiscuous gene. Once broken, it can reconnect with any of more than 40 other genes in a translocation, a process that involves an exchange of DNA between two chromosomes. Extensive recombinations usually cause cell death; but subtle translocations involving MLL can result in the rapid, uncontrolled cell division seen in leukemia.	topic_ll
75184	3	355599	5	NULL	NULL	0	NULL	statement 2	Process		occurs during					translocation	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	MLL is a promiscuous gene. Once broken, it can reconnect with any of more than 40 other genes in a translocation, a process that involves an exchange of DNA between two chromosomes. Extensive recombinations usually cause cell death; but subtle translocations involving MLL can result in the rapid, uncontrolled cell division seen in leukemia.	topic_ll
75185	4	355599	5	NULL	NULL	0	NULL	DNA	NucleicAcid		is exchanged between					chromosomes	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	MLL is a promiscuous gene. Once broken, it can reconnect with any of more than 40 other genes in a translocation, a process that involves an exchange of DNA between two chromosomes. Extensive recombinations usually cause cell death; but subtle translocations involving MLL can result in the rapid, uncontrolled cell division seen in leukemia.	topic_ll
75186	5	355599	5	NULL	NULL	0	NULL	translocation	Process		involves					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	MLL is a promiscuous gene. Once broken, it can reconnect with any of more than 40 other genes in a translocation, a process that involves an exchange of DNA between two chromosomes. Extensive recombinations usually cause cell death; but subtle translocations involving MLL can result in the rapid, uncontrolled cell division seen in leukemia.	topic_ll
75187	6	355599	5	NULL	NULL	0	NULL	recombinations	Process	extensive	cause		usually			cell death	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	MLL is a promiscuous gene. Once broken, it can reconnect with any of more than 40 other genes in a translocation, a process that involves an exchange of DNA between two chromosomes. Extensive recombinations usually cause cell death; but subtle translocations involving MLL can result in the rapid, uncontrolled cell division seen in leukemia.	topic_ll
75188	7	355599	5	NULL	NULL	0	NULL	translocation	Process	subtle	involve					MLL	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	MLL is a promiscuous gene. Once broken, it can reconnect with any of more than 40 other genes in a translocation, a process that involves an exchange of DNA between two chromosomes. Extensive recombinations usually cause cell death; but subtle translocations involving MLL can result in the rapid, uncontrolled cell division seen in leukemia.	topic_ll
75189	8	355599	5	NULL	NULL	0	NULL	statement 7	Process		results in					cell division	Process	repid;;uncontrolled			NULL		0	NULL	NULL	NULL	NULL	NULL	MLL is a promiscuous gene. Once broken, it can reconnect with any of more than 40 other genes in a translocation, a process that involves an exchange of DNA between two chromosomes. Extensive recombinations usually cause cell death; but subtle translocations involving MLL can result in the rapid, uncontrolled cell division seen in leukemia.	topic_ll
75190	9	355599	5	NULL	NULL	0	NULL	statement 8	Process		is seen in					leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	MLL is a promiscuous gene. Once broken, it can reconnect with any of more than 40 other genes in a translocation, a process that involves an exchange of DNA between two chromosomes. Extensive recombinations usually cause cell death; but subtle translocations involving MLL can result in the rapid, uncontrolled cell division seen in leukemia.	topic_ll
75191	1	355600	5	NULL	NULL	0	NULL	VP16	Chemical		is a type of					anti-cancer drug	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA damage seen after exposure to either bioflavonoids or to anti-cancer drugs VP16 or doxorubicin (Dox) was identical, affecting one small region of the MLL gene. Although most adult leukemias involving MLL affect a different part of the gene, the breakpoints found in infant leukemias and secondary leukemias occur predominantly in the small region altered by the bioflavonoids.	topic_ll
75192	2	355600	5	NULL	NULL	0	NULL	Dox	Chemical		is					doxorubicin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA damage seen after exposure to either bioflavonoids or to anti-cancer drugs VP16 or doxorubicin (Dox) was identical, affecting one small region of the MLL gene. Although most adult leukemias involving MLL affect a different part of the gene, the breakpoints found in infant leukemias and secondary leukemias occur predominantly in the small region altered by the bioflavonoids.	topic_ll
75193	3	355600	5	NULL	NULL	0	NULL	doxorubicin	Chemical		is a type of					anti-cancer drug	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA damage seen after exposure to either bioflavonoids or to anti-cancer drugs VP16 or doxorubicin (Dox) was identical, affecting one small region of the MLL gene. Although most adult leukemias involving MLL affect a different part of the gene, the breakpoints found in infant leukemias and secondary leukemias occur predominantly in the small region altered by the bioflavonoids.	topic_ll
75194	4	355600	5	NULL	NULL	0	NULL	bioflavonoids	Chemical	exposure	leads to					DNA damage	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA damage seen after exposure to either bioflavonoids or to anti-cancer drugs VP16 or doxorubicin (Dox) was identical, affecting one small region of the MLL gene. Although most adult leukemias involving MLL affect a different part of the gene, the breakpoints found in infant leukemias and secondary leukemias occur predominantly in the small region altered by the bioflavonoids.	topic_ll
75195	5	355600	5	NULL	NULL	0	NULL	VP16	Chemical	exposure	leads to					DNA damage	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA damage seen after exposure to either bioflavonoids or to anti-cancer drugs VP16 or doxorubicin (Dox) was identical, affecting one small region of the MLL gene. Although most adult leukemias involving MLL affect a different part of the gene, the breakpoints found in infant leukemias and secondary leukemias occur predominantly in the small region altered by the bioflavonoids.	topic_ll
75196	6	355600	5	NULL	NULL	0	NULL	doxorubicin	Chemical	exposure	leads to					DNA damage	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA damage seen after exposure to either bioflavonoids or to anti-cancer drugs VP16 or doxorubicin (Dox) was identical, affecting one small region of the MLL gene. Although most adult leukemias involving MLL affect a different part of the gene, the breakpoints found in infant leukemias and secondary leukemias occur predominantly in the small region altered by the bioflavonoids.	topic_ll
75197	7	355600	5	NULL	NULL	0	NULL	statement 4	Process		identical to					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA damage seen after exposure to either bioflavonoids or to anti-cancer drugs VP16 or doxorubicin (Dox) was identical, affecting one small region of the MLL gene. Although most adult leukemias involving MLL affect a different part of the gene, the breakpoints found in infant leukemias and secondary leukemias occur predominantly in the small region altered by the bioflavonoids.	topic_ll
75198	8	355600	5	NULL	NULL	0	NULL	statement 5	Process		identical to					statement 6	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA damage seen after exposure to either bioflavonoids or to anti-cancer drugs VP16 or doxorubicin (Dox) was identical, affecting one small region of the MLL gene. Although most adult leukemias involving MLL affect a different part of the gene, the breakpoints found in infant leukemias and secondary leukemias occur predominantly in the small region altered by the bioflavonoids.	topic_ll
75199	9	355600	5	NULL	NULL	0	NULL	statement 4	Process		affect					MLL gene	GP	small region of			NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA damage seen after exposure to either bioflavonoids or to anti-cancer drugs VP16 or doxorubicin (Dox) was identical, affecting one small region of the MLL gene. Although most adult leukemias involving MLL affect a different part of the gene, the breakpoints found in infant leukemias and secondary leukemias occur predominantly in the small region altered by the bioflavonoids.	topic_ll
75200	10	355600	5	NULL	NULL	0	NULL	statement 5	Process		affect					MLL gene	GP	small region of			NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA damage seen after exposure to either bioflavonoids or to anti-cancer drugs VP16 or doxorubicin (Dox) was identical, affecting one small region of the MLL gene. Although most adult leukemias involving MLL affect a different part of the gene, the breakpoints found in infant leukemias and secondary leukemias occur predominantly in the small region altered by the bioflavonoids.	topic_ll
75201	11	355600	5	NULL	NULL	0	NULL	statement 6	Process		affect					MLL gene	GP	small region of			NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA damage seen after exposure to either bioflavonoids or to anti-cancer drugs VP16 or doxorubicin (Dox) was identical, affecting one small region of the MLL gene. Although most adult leukemias involving MLL affect a different part of the gene, the breakpoints found in infant leukemias and secondary leukemias occur predominantly in the small region altered by the bioflavonoids.	topic_ll
75224	12	355600	5	NULL	NULL	NULL	NULL	leukemia	MedicalFinding	adult	involve					MLL gene	GP	damage of;;different part of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	The DNA damage seen after exposure to either bioflavonoids or to anti-cancer drugs VP16 or doxorubicin (Dox) was identical, affecting one small region of the MLL gene. Although most adult leukemias involving MLL affect a different part of the gene, the breakpoints found in infant leukemias and secondary leukemias occur predominantly in the small region altered by the bioflavonoids.	topic_ll
75225	13	355600	5	NULL	NULL	0	NULL	statement 9	Process		leads to					leukemia	MedicalFinding	infant			NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA damage seen after exposure to either bioflavonoids or to anti-cancer drugs VP16 or doxorubicin (Dox) was identical, affecting one small region of the MLL gene. Although most adult leukemias involving MLL affect a different part of the gene, the breakpoints found in infant leukemias and secondary leukemias occur predominantly in the small region altered by the bioflavonoids.	topic_ll
75226	14	355600	5	NULL	NULL	0	NULL	statement 9	Process		leads to					leukemia	MedicalFinding	secondary			NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA damage seen after exposure to either bioflavonoids or to anti-cancer drugs VP16 or doxorubicin (Dox) was identical, affecting one small region of the MLL gene. Although most adult leukemias involving MLL affect a different part of the gene, the breakpoints found in infant leukemias and secondary leukemias occur predominantly in the small region altered by the bioflavonoids.	topic_ll
75227	1	355601	5	NULL	NULL	0	NULL	bioflavonoids	Chemical		cause					DNA damage	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Some bioflavonoids were as active in causing DNA damage as the powerful anti-cancer drug etoposide (VP16), which has been tied to secondary leukemias--cancers of the bone marrow that result from previous anti-cancer therapy.	topic_ll
75228	2	355601	5	NULL	NULL	0	NULL	VP16	Chemical		cause					DNA damage	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Some bioflavonoids were as active in causing DNA damage as the powerful anti-cancer drug etoposide (VP16), which has been tied to secondary leukemias--cancers of the bone marrow that result from previous anti-cancer therapy.	topic_ll
75229	3	355601	5	NULL	NULL	0	NULL	bioflavonoids	Chemical		is as active as					VP16	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Some bioflavonoids were as active in causing DNA damage as the powerful anti-cancer drug etoposide (VP16), which has been tied to secondary leukemias--cancers of the bone marrow that result from previous anti-cancer therapy.	topic_ll
75230	4	355601	5	NULL	NULL	0	NULL	VP16	Chemical		is also known as					etoposide	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Some bioflavonoids were as active in causing DNA damage as the powerful anti-cancer drug etoposide (VP16), which has been tied to secondary leukemias--cancers of the bone marrow that result from previous anti-cancer therapy.	topic_ll
75231	5	355601	5	NULL	NULL	0	NULL	etoposide	Chemical		is a type of					anti-cancer drug	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Some bioflavonoids were as active in causing DNA damage as the powerful anti-cancer drug etoposide (VP16), which has been tied to secondary leukemias--cancers of the bone marrow that result from previous anti-cancer therapy.	topic_ll
75232	6	355601	5	NULL	NULL	0	NULL	VP16	Chemical		is associated with					leukemia	MedicalFinding	secondary			NULL		0	NULL	NULL	NULL	NULL	NULL	Some bioflavonoids were as active in causing DNA damage as the powerful anti-cancer drug etoposide (VP16), which has been tied to secondary leukemias--cancers of the bone marrow that result from previous anti-cancer therapy.	topic_ll
75233	7	355601	5	NULL	NULL	0	NULL	bone marrow cancer	MedicalFinding		results from					anti-cancer therapy	MedicalProcedure	previous			NULL		0	NULL	NULL	NULL	NULL	NULL	Some bioflavonoids were as active in causing DNA damage as the powerful anti-cancer drug etoposide (VP16), which has been tied to secondary leukemias--cancers of the bone marrow that result from previous anti-cancer therapy.	topic_ll
75235	8	355601	5	NULL	NULL	0	NULL	statement 7	Process		is a type of					leukemia	MedicalFinding	secondary			NULL		0	NULL	NULL	NULL	NULL	NULL	Some bioflavonoids were as active in causing DNA damage as the powerful anti-cancer drug etoposide (VP16), which has been tied to secondary leukemias--cancers of the bone marrow that result from previous anti-cancer therapy.	topic_ll
75239	1	355602	5	NULL	NULL	0	NULL	leukemia	MedicalFinding	childhood	is a type of					cancer	MedicalFinding	childhood			NULL		0	NULL	NULL	NULL	NULL	NULL	A new study led by researchers at the University of California, Berkeley, suggests that women who eat more vegetables, fruit and foods containing protein before pregnancy may have a lower risk of having a child who develops leukemia, the most common childhood cancer in the United States. 	topic_ll
75240	2	355602	5	NULL	NULL	0	NULL	statement 1	Process		occurs in					United States	GeographicLocation				NULL		0	NULL	NULL	NULL	NULL	NULL	A new study led by researchers at the University of California, Berkeley, suggests that women who eat more vegetables, fruit and foods containing protein before pregnancy may have a lower risk of having a child who develops leukemia, the most common childhood cancer in the United States. 	topic_ll
75376	1	355603	5	NULL	NULL	0	NULL	MLL	GP		is translocated in					ALL infants	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that 74% of infants with ALL had an MLL translocation; the most common partner genes were AF4, ENL, and AF9. Both AF4 (located on chromosome 4) and ENL (located on chromosome 19) negatively affected patient survival, whereas AF9 (located on chromosome 9) was associated with better survival.	topic_ll
75377	2	355603	5	NULL	NULL	0	NULL	AF4	GP		is a partner of					MLL	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that 74% of infants with ALL had an MLL translocation; the most common partner genes were AF4, ENL, and AF9. Both AF4 (located on chromosome 4) and ENL (located on chromosome 19) negatively affected patient survival, whereas AF9 (located on chromosome 9) was associated with better survival.	topic_ll
75378	3	355603	5	NULL	NULL	0	NULL	ENL	GP		is a partner of					MLL	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that 74% of infants with ALL had an MLL translocation; the most common partner genes were AF4, ENL, and AF9. Both AF4 (located on chromosome 4) and ENL (located on chromosome 19) negatively affected patient survival, whereas AF9 (located on chromosome 9) was associated with better survival.	topic_ll
75379	4	355603	5	NULL	NULL	0	NULL	AF9	GP		is a partner of					MLL	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that 74% of infants with ALL had an MLL translocation; the most common partner genes were AF4, ENL, and AF9. Both AF4 (located on chromosome 4) and ENL (located on chromosome 19) negatively affected patient survival, whereas AF9 (located on chromosome 9) was associated with better survival.	topic_ll
75380	5	355603	5	NULL	NULL	0	NULL	AF4	GP		is located on					chromosome 4	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that 74% of infants with ALL had an MLL translocation; the most common partner genes were AF4, ENL, and AF9. Both AF4 (located on chromosome 4) and ENL (located on chromosome 19) negatively affected patient survival, whereas AF9 (located on chromosome 9) was associated with better survival.	topic_ll
75381	6	355603	5	NULL	NULL	0	NULL	ENL	GP		is located on					chromosome 19	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that 74% of infants with ALL had an MLL translocation; the most common partner genes were AF4, ENL, and AF9. Both AF4 (located on chromosome 4) and ENL (located on chromosome 19) negatively affected patient survival, whereas AF9 (located on chromosome 9) was associated with better survival.	topic_ll
75382	7	355603	5	NULL	NULL	0	NULL	AF4	GP		affects		negatively			ALL infants	GroupOfPeople	survival of			NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that 74% of infants with ALL had an MLL translocation; the most common partner genes were AF4, ENL, and AF9. Both AF4 (located on chromosome 4) and ENL (located on chromosome 19) negatively affected patient survival, whereas AF9 (located on chromosome 9) was associated with better survival.	topic_ll
75383	8	355603	5	NULL	NULL	0	NULL	ENL	GP		affects		negatively			ALL infants	GroupOfPeople	survival of			NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that 74% of infants with ALL had an MLL translocation; the most common partner genes were AF4, ENL, and AF9. Both AF4 (located on chromosome 4) and ENL (located on chromosome 19) negatively affected patient survival, whereas AF9 (located on chromosome 9) was associated with better survival.	topic_ll
75384	9	355603	5	NULL	NULL	0	NULL	AF9	GP		is located on					chromosome 9	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that 74% of infants with ALL had an MLL translocation; the most common partner genes were AF4, ENL, and AF9. Both AF4 (located on chromosome 4) and ENL (located on chromosome 19) negatively affected patient survival, whereas AF9 (located on chromosome 9) was associated with better survival.	topic_ll
75385	10	355603	5	NULL	NULL	0	NULL	AF9	GP		is associated with					ALL infants	GroupOfPeople	better survival of			NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that 74% of infants with ALL had an MLL translocation; the most common partner genes were AF4, ENL, and AF9. Both AF4 (located on chromosome 4) and ENL (located on chromosome 19) negatively affected patient survival, whereas AF9 (located on chromosome 9) was associated with better survival.	topic_ll
75386	1	355604	5	NULL	NULL	0	NULL	MLL	GP		fuse with					AF4	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	that the less favorable fusion of MLL with AF4 was associated with a higher white count, and that the fusion of MLL with AF9 was associated with a lower white blood cell count.	topic_ll
75387	2	355604	5	NULL	NULL	NULL	NULL	statement 1	Process		is associated with					white blood cell count	MedicalProcedure	higher			NULL		NULL	NULL	NULL	NULL	NULL	NULL	that the less favorable fusion of MLL with AF4 was associated with a higher white count, and that the fusion of MLL with AF9 was associated with a lower white blood cell count.	topic_ll
75388	3	355604	5	NULL	NULL	0	NULL	MLL	GP		fuse with					AF9	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	that the less favorable fusion of MLL with AF4 was associated with a higher white count, and that the fusion of MLL with AF9 was associated with a lower white blood cell count.	topic_ll
75389	4	355604	5	NULL	NULL	0	NULL	statement 3	Process		is associated with					white blood cell count	MedicalProcedure	lower			NULL		0	NULL	NULL	NULL	NULL	NULL	that the less favorable fusion of MLL with AF4 was associated with a higher white count, and that the fusion of MLL with AF9 was associated with a lower white blood cell count.	topic_ll
75390	1	355606	5	NULL	NULL	0	NULL	MLL	GP		is translocated in					ALL infants	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that 74% of infants with ALL had an MLL translocation -  the most common partner genes were AF4, ENL, and AF9.	topic_ll
75391	2	355606	5	NULL	NULL	0	NULL	AF4	GP		is a partner of					MLL	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that 74% of infants with ALL had an MLL translocation -  the most common partner genes were AF4, ENL, and AF9.	topic_ll
75392	3	355606	5	NULL	NULL	0	NULL	ENL	GP		is a partner of					MLL	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that 74% of infants with ALL had an MLL translocation -  the most common partner genes were AF4, ENL, and AF9.	topic_ll
75393	4	355606	5	NULL	NULL	0	NULL	AF9	GP		is a partner of					MLL	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that 74% of infants with ALL had an MLL translocation -  the most common partner genes were AF4, ENL, and AF9.	topic_ll
75394	1	355607	5	NULL	NULL	0	NULL	acute lymphoblastic leukemia	MedicalFinding	few cases of	is associated with					Down syndrome	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Acute lymphoblastic leukemia: Although a few cases are associated with inherited genetic syndromes (ie, Down syndrome, Bloom syndrome, Fanconi anemia), the cause remains largely unknown. Many environmental factors (ie, exposure to ionizing radiation and electromagnetic fields, parental use of alcohol and tobacco) have been investigated as potential risk factors, but none has been definitively shown to cause acute lymphoblastic leukemia. 	topic_ll
75395	2	355607	5	NULL	NULL	0	NULL	acute lymphoblastic leukemia	MedicalFinding	few cases of	is associated with					Bloom syndrome	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Acute lymphoblastic leukemia: Although a few cases are associated with inherited genetic syndromes (ie, Down syndrome, Bloom syndrome, Fanconi anemia), the cause remains largely unknown. Many environmental factors (ie, exposure to ionizing radiation and electromagnetic fields, parental use of alcohol and tobacco) have been investigated as potential risk factors, but none has been definitively shown to cause acute lymphoblastic leukemia. 	topic_ll
75396	3	355607	5	NULL	NULL	0	NULL	acute lymphoblastic leukemia	MedicalFinding		is associated with					Fanconi anemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Acute lymphoblastic leukemia: Although a few cases are associated with inherited genetic syndromes (ie, Down syndrome, Bloom syndrome, Fanconi anemia), the cause remains largely unknown. Many environmental factors (ie, exposure to ionizing radiation and electromagnetic fields, parental use of alcohol and tobacco) have been investigated as potential risk factors, but none has been definitively shown to cause acute lymphoblastic leukemia. 	topic_ll
75397	4	355607	5	NULL	NULL	0	NULL	Down syndrome	MedicalFinding		is a type of					inherited genetic syndrome	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Acute lymphoblastic leukemia: Although a few cases are associated with inherited genetic syndromes (ie, Down syndrome, Bloom syndrome, Fanconi anemia), the cause remains largely unknown. Many environmental factors (ie, exposure to ionizing radiation and electromagnetic fields, parental use of alcohol and tobacco) have been investigated as potential risk factors, but none has been definitively shown to cause acute lymphoblastic leukemia. 	topic_ll
75398	5	355607	5	NULL	NULL	0	NULL	Bloom syndrome	MedicalFinding		is a type of					inherited genetic syndrome	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Acute lymphoblastic leukemia: Although a few cases are associated with inherited genetic syndromes (ie, Down syndrome, Bloom syndrome, Fanconi anemia), the cause remains largely unknown. Many environmental factors (ie, exposure to ionizing radiation and electromagnetic fields, parental use of alcohol and tobacco) have been investigated as potential risk factors, but none has been definitively shown to cause acute lymphoblastic leukemia. 	topic_ll
75399	6	355607	5	NULL	NULL	0	NULL	Fanconi anemia	MedicalFinding		is a type of					inherited genetic syndrome	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Acute lymphoblastic leukemia: Although a few cases are associated with inherited genetic syndromes (ie, Down syndrome, Bloom syndrome, Fanconi anemia), the cause remains largely unknown. Many environmental factors (ie, exposure to ionizing radiation and electromagnetic fields, parental use of alcohol and tobacco) have been investigated as potential risk factors, but none has been definitively shown to cause acute lymphoblastic leukemia. 	topic_ll
75400	7	355607	5	NULL	NULL	0	NULL	ionizing radiation	PhysicalPhenomenon	exposure to	does not cause					acute lymphoblastic leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Acute lymphoblastic leukemia: Although a few cases are associated with inherited genetic syndromes (ie, Down syndrome, Bloom syndrome, Fanconi anemia), the cause remains largely unknown. Many environmental factors (ie, exposure to ionizing radiation and electromagnetic fields, parental use of alcohol and tobacco) have been investigated as potential risk factors, but none has been definitively shown to cause acute lymphoblastic leukemia. 	topic_ll
75401	8	355607	5	NULL	NULL	0	NULL	electromagnetic fields	PhysicalPhenomenon	exposure to	does not cause					acute lymphoblastic leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Acute lymphoblastic leukemia: Although a few cases are associated with inherited genetic syndromes (ie, Down syndrome, Bloom syndrome, Fanconi anemia), the cause remains largely unknown. Many environmental factors (ie, exposure to ionizing radiation and electromagnetic fields, parental use of alcohol and tobacco) have been investigated as potential risk factors, but none has been definitively shown to cause acute lymphoblastic leukemia. 	topic_ll
75402	9	355607	5	NULL	NULL	0	NULL	alcohol	Chemical	parental use of	does not cause					acute lymphoblastic leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Acute lymphoblastic leukemia: Although a few cases are associated with inherited genetic syndromes (ie, Down syndrome, Bloom syndrome, Fanconi anemia), the cause remains largely unknown. Many environmental factors (ie, exposure to ionizing radiation and electromagnetic fields, parental use of alcohol and tobacco) have been investigated as potential risk factors, but none has been definitively shown to cause acute lymphoblastic leukemia. 	topic_ll
75403	10	355607	5	NULL	NULL	0	NULL	tobacco	Chemical	parental use of	does not cause					acute lymphoblastic leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Acute lymphoblastic leukemia: Although a few cases are associated with inherited genetic syndromes (ie, Down syndrome, Bloom syndrome, Fanconi anemia), the cause remains largely unknown. Many environmental factors (ie, exposure to ionizing radiation and electromagnetic fields, parental use of alcohol and tobacco) have been investigated as potential risk factors, but none has been definitively shown to cause acute lymphoblastic leukemia. 	topic_ll
75404	11	355607	5	NULL	NULL	0	NULL	ionizing radiation	PhysicalPhenomenon		is a type of					environmental factor	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	NULL	NULL	Acute lymphoblastic leukemia: Although a few cases are associated with inherited genetic syndromes (ie, Down syndrome, Bloom syndrome, Fanconi anemia), the cause remains largely unknown. Many environmental factors (ie, exposure to ionizing radiation and electromagnetic fields, parental use of alcohol and tobacco) have been investigated as potential risk factors, but none has been definitively shown to cause acute lymphoblastic leukemia. 	topic_ll
75405	12	355607	5	NULL	NULL	0	NULL	electromagnetic fields	PhysicalPhenomenon		is a type of					environmental factor	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	NULL	NULL	Acute lymphoblastic leukemia: Although a few cases are associated with inherited genetic syndromes (ie, Down syndrome, Bloom syndrome, Fanconi anemia), the cause remains largely unknown. Many environmental factors (ie, exposure to ionizing radiation and electromagnetic fields, parental use of alcohol and tobacco) have been investigated as potential risk factors, but none has been definitively shown to cause acute lymphoblastic leukemia. 	topic_ll
75406	13	355607	5	NULL	NULL	0	NULL	alcohol	Chemical		is a type of					environmental factor	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Acute lymphoblastic leukemia: Although a few cases are associated with inherited genetic syndromes (ie, Down syndrome, Bloom syndrome, Fanconi anemia), the cause remains largely unknown. Many environmental factors (ie, exposure to ionizing radiation and electromagnetic fields, parental use of alcohol and tobacco) have been investigated as potential risk factors, but none has been definitively shown to cause acute lymphoblastic leukemia. 	topic_ll
75407	14	355607	5	NULL	NULL	0	NULL	tobacco	Chemical		is a type of					environmental factor	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Acute lymphoblastic leukemia: Although a few cases are associated with inherited genetic syndromes (ie, Down syndrome, Bloom syndrome, Fanconi anemia), the cause remains largely unknown. Many environmental factors (ie, exposure to ionizing radiation and electromagnetic fields, parental use of alcohol and tobacco) have been investigated as potential risk factors, but none has been definitively shown to cause acute lymphoblastic leukemia. 	topic_ll
75470	1	355608	5	NULL	NULL	0	NULL	Wiskott-Aldrich syndrome	MedicalFinding		is a type of					congenital immunodeficiencies	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Acute lymphoblastic leukemia may also occur in children with various congenital immunodeficiencies (ie, Wiskott-Aldrich syndrome, congenital hypogammaglobulinemia, ataxia-telangiectasia) that have an increased predisposition to develop lymphoid malignancies.	topic_ll
75471	2	355608	5	NULL	NULL	0	NULL	congenital hypogammaglobulinemia	MedicalFinding		is a type of					congenital immunodeficiencies	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Acute lymphoblastic leukemia may also occur in children with various congenital immunodeficiencies (ie, Wiskott-Aldrich syndrome, congenital hypogammaglobulinemia, ataxia-telangiectasia) that have an increased predisposition to develop lymphoid malignancies.	topic_ll
75473	3	355608	5	NULL	NULL	0	NULL	ataxia-telangiectasia	MedicalFinding		is a type of					congenital immunodeficiencies	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Acute lymphoblastic leukemia may also occur in children with various congenital immunodeficiencies (ie, Wiskott-Aldrich syndrome, congenital hypogammaglobulinemia, ataxia-telangiectasia) that have an increased predisposition to develop lymphoid malignancies.	topic_ll
75474	4	355608	5	NULL	NULL	0	NULL	children	GroupOfPeople		suffer from					statement 1	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Acute lymphoblastic leukemia may also occur in children with various congenital immunodeficiencies (ie, Wiskott-Aldrich syndrome, congenital hypogammaglobulinemia, ataxia-telangiectasia) that have an increased predisposition to develop lymphoid malignancies.	topic_ll
75475	5	355608	5	NULL	NULL	NULL	NULL	children	GroupOfPeople		suffer from					statement 2	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Acute lymphoblastic leukemia may also occur in children with various congenital immunodeficiencies (ie, Wiskott-Aldrich syndrome, congenital hypogammaglobulinemia, ataxia-telangiectasia) that have an increased predisposition to develop lymphoid malignancies.	topic_ll
75476	6	355608	5	NULL	NULL	0	NULL	children	GroupOfPeople		suffer from					statement 3	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Acute lymphoblastic leukemia may also occur in children with various congenital immunodeficiencies (ie, Wiskott-Aldrich syndrome, congenital hypogammaglobulinemia, ataxia-telangiectasia) that have an increased predisposition to develop lymphoid malignancies.	topic_ll
75477	7	355608	5	NULL	NULL	0	NULL	acute lymphoblastic leukemia	MedicalFinding		occurs in		may			statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Acute lymphoblastic leukemia may also occur in children with various congenital immunodeficiencies (ie, Wiskott-Aldrich syndrome, congenital hypogammaglobulinemia, ataxia-telangiectasia) that have an increased predisposition to develop lymphoid malignancies.	topic_ll
75478	8	355608	5	NULL	NULL	0	NULL	acute lymphoblastic leukemia	MedicalFinding		occurs in		may			statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Acute lymphoblastic leukemia may also occur in children with various congenital immunodeficiencies (ie, Wiskott-Aldrich syndrome, congenital hypogammaglobulinemia, ataxia-telangiectasia) that have an increased predisposition to develop lymphoid malignancies.	topic_ll
75479	9	355608	5	NULL	NULL	0	NULL	acute lymphoblastic leukemia	MedicalFinding		occurs in		may			statement 6	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Acute lymphoblastic leukemia may also occur in children with various congenital immunodeficiencies (ie, Wiskott-Aldrich syndrome, congenital hypogammaglobulinemia, ataxia-telangiectasia) that have an increased predisposition to develop lymphoid malignancies.	topic_ll
75480	10	355608	5	NULL	NULL	0	NULL	statement 1	MedicalFinding		predisposed to develop		increase			lymphoid malignancies	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Acute lymphoblastic leukemia may also occur in children with various congenital immunodeficiencies (ie, Wiskott-Aldrich syndrome, congenital hypogammaglobulinemia, ataxia-telangiectasia) that have an increased predisposition to develop lymphoid malignancies.	topic_ll
75481	11	355608	5	NULL	NULL	NULL	NULL	statement 2	MedicalFinding		predisposed to develop		increase			lymphoid malignancies	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Acute lymphoblastic leukemia may also occur in children with various congenital immunodeficiencies (ie, Wiskott-Aldrich syndrome, congenital hypogammaglobulinemia, ataxia-telangiectasia) that have an increased predisposition to develop lymphoid malignancies.	topic_ll
75482	12	355608	5	NULL	NULL	0	NULL	statement 3	MedicalFinding		predisposed to develop		increase			lymphoid malignancies	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Acute lymphoblastic leukemia may also occur in children with various congenital immunodeficiencies (ie, Wiskott-Aldrich syndrome, congenital hypogammaglobulinemia, ataxia-telangiectasia) that have an increased predisposition to develop lymphoid malignancies.	topic_ll
75484	1	355609	5	NULL	NULL	0	NULL	virus	Organism		is linked to		may be			leukemia	MedicalFinding	development of			NULL		0	NULL	NULL	NULL	NULL	NULL	Various viruses may be linked to the development of leukemia, particularly when prenatal viral exposure occurs in mothers recently infected with influenza or varicella. 	topic_ll
75485	2	355609	5	NULL	NULL	0	NULL	mothers	GroupOfPeople		infected with		recently			influenza	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Various viruses may be linked to the development of leukemia, particularly when prenatal viral exposure occurs in mothers recently infected with influenza or varicella. 	topic_ll
75486	3	355609	5	NULL	NULL	0	NULL	mothers	GroupOfPeople		infected with		recently			varicella	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Various viruses may be linked to the development of leukemia, particularly when prenatal viral exposure occurs in mothers recently infected with influenza or varicella. 	topic_ll
75488	4	355609	5	NULL	NULL	0	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Various viruses may be linked to the development of leukemia, particularly when prenatal viral exposure occurs in mothers recently infected with influenza or varicella. 	topic_ll
75493	5	355609	5	NULL	NULL	0	NULL	statement 2	Process		is exposed to		prenatally			virus	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Various viruses may be linked to the development of leukemia, particularly when prenatal viral exposure occurs in mothers recently infected with influenza or varicella. 	topic_ll
75495	6	355609	5	NULL	NULL	0	NULL	statement 5	Process		is associated with					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Various viruses may be linked to the development of leukemia, particularly when prenatal viral exposure occurs in mothers recently infected with influenza or varicella. 	topic_ll
75496	7	355609	5	NULL	NULL	0	NULL	statement 3	Process		is exposed to		prenatally			virus	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Various viruses may be linked to the development of leukemia, particularly when prenatal viral exposure occurs in mothers recently infected with influenza or varicella. 	topic_ll
75497	8	355609	5	NULL	NULL	0	NULL	statement 7	Process		is associated with					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Various viruses may be linked to the development of leukemia, particularly when prenatal viral exposure occurs in mothers recently infected with influenza or varicella. 	topic_ll
76484	1	355610	11	NULL	NULL	0	NULL	Sulfonamide	Chemical		is also known as					sulfa drugs	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfonamide is the basis of several groups of drugs. The original antibacterial sulfonamides (sometimes called simply sulfa drugs) are synthetic antimicrobial agents that contain the sulfonamide group	topic_mrs
76485	2	355610	11	NULL	NULL	0	NULL	Sulfonamide	Chemical		is a type of 					 synthetic antimicrobial agent	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfonamide is the basis of several groups of drugs. The original antibacterial sulfonamides (sometimes called simply sulfa drugs) are synthetic antimicrobial agents that contain the sulfonamide group	topic_mrs
75614	1	355611	11	NULL	NULL	0	NULL	Staphylococcus aureus 	Organism		causes					skin and soft tissue infections	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Staphylococcus aureus skin and soft tissue infections (SSTI) in outpatients in Illinois, in the setting of increasing levels of community-associated methicillin resistant S. aureus (CA-MRSA).	topic_mrs
75615	2	355611	11	NULL	NULL	0	NULL	skin and soft tissue infections	MedicalFinding		is					SSTI	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Staphylococcus aureus skin and soft tissue infections (SSTI) in outpatients in Illinois, in the setting of increasing levels of community-associated methicillin resistant S. aureus (CA-MRSA).	topic_mrs
76486	1	355612	11	NULL	NULL	0	NULL	cutaneous abscess	MedicalFinding		treats by 					 incision	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	For a cutaneous abscess, incision and drainage is the primary treatment. For simple abscesses or boils, incision and drainage alone is likely to be adequate, but additional data are needed to further deﬁne the role of antibiotics, if any, in this setting.	topic_mrs
76487	2	355612	11	NULL	NULL	0	NULL	cutaneous abscess	MedicalFinding		treats by 					drainage	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	For a cutaneous abscess, incision and drainage is the primary treatment. For simple abscesses or boils, incision and drainage alone is likely to be adequate, but additional data are needed to further deﬁne the role of antibiotics, if any, in this setting.	topic_mrs
76488	3	355612	11	NULL	NULL	0	NULL	statement 1	Process		occurs along with					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	For a cutaneous abscess, incision and drainage is the primary treatment. For simple abscesses or boils, incision and drainage alone is likely to be adequate, but additional data are needed to further deﬁne the role of antibiotics, if any, in this setting.	topic_mrs
76489	4	355612	11	NULL	NULL	0	NULL	 simple abscesses	MedicalFinding		treats by 					incision	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	For a cutaneous abscess, incision and drainage is the primary treatment. For simple abscesses or boils, incision and drainage alone is likely to be adequate, but additional data are needed to further deﬁne the role of antibiotics, if any, in this setting.	topic_mrs
76490	5	355612	11	NULL	NULL	0	NULL	 simple abscesses	MedicalFinding		treats by 					drainage	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	For a cutaneous abscess, incision and drainage is the primary treatment. For simple abscesses or boils, incision and drainage alone is likely to be adequate, but additional data are needed to further deﬁne the role of antibiotics, if any, in this setting.	topic_mrs
76491	6	355612	11	NULL	NULL	0	NULL	statement 4	Process		occurs along with					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	For a cutaneous abscess, incision and drainage is the primary treatment. For simple abscesses or boils, incision and drainage alone is likely to be adequate, but additional data are needed to further deﬁne the role of antibiotics, if any, in this setting.	topic_mrs
76492	7	355612	11	NULL	NULL	0	NULL	boils	MedicalFinding		treats by 					incision	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	For a cutaneous abscess, incision and drainage is the primary treatment. For simple abscesses or boils, incision and drainage alone is likely to be adequate, but additional data are needed to further deﬁne the role of antibiotics, if any, in this setting.	topic_mrs
76493	8	355612	11	NULL	NULL	0	NULL	boils	MedicalFinding		treats by 					drainage	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	For a cutaneous abscess, incision and drainage is the primary treatment. For simple abscesses or boils, incision and drainage alone is likely to be adequate, but additional data are needed to further deﬁne the role of antibiotics, if any, in this setting.	topic_mrs
76494	9	355612	11	NULL	NULL	0	NULL	statement 7	Process		occurs along with					statement 8	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	For a cutaneous abscess, incision and drainage is the primary treatment. For simple abscesses or boils, incision and drainage alone is likely to be adequate, but additional data are needed to further deﬁne the role of antibiotics, if any, in this setting.	topic_mrs
76495	1	355614	11	NULL	NULL	0	NULL	mupirocin	Chemical		treats					Nasal decolonization	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nasal decolonization with mupirocin twice daily for 5–10 days	topic_mrs
76496	1	355615	11	NULL	NULL	0	NULL	mupirocin	Chemical		treats					Nasal decolonization	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nasal decolonization with mupirocin twice daily for 5–10 days and topical body decolonization regimens with a skin antiseptic solution (eg, chlorhexidine) for 5–14 days or dilute bleach baths.	topic_mrs
76497	2	355615	11	NULL	NULL	0	NULL	chlorhexidine	Chemical		is a type of 					skin antiseptic solution	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Nasal decolonization with mupirocin twice daily for 5–10 days and topical body decolonization regimens with a skin antiseptic solution (eg, chlorhexidine) for 5–14 days or dilute bleach baths.	topic_mrs
76498	1	355616	11	NULL	NULL	0	NULL	recurrent skin infections	Process		treats by 					Dilute bleach baths	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Dilute bleach baths have long been recommended to help children with recurrent skin infections, especially those with hard to control eczema and/or MRSA (Methicillin resistant Staphylococcus aureus) infections.	topic_mrs
76499	2	355616	11	NULL	NULL	0	NULL	Methicillin resistant Staphylococcus aureus	Organism		is					MRSA	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Dilute bleach baths have long been recommended to help children with recurrent skin infections, especially those with hard to control eczema and/or MRSA (Methicillin resistant Staphylococcus aureus) infections.	topic_mrs
76500	3	355616	11	NULL	NULL	0	NULL	eczema	MedicalFinding		is a type of 					recurrent skin infections	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Dilute bleach baths have long been recommended to help children with recurrent skin infections, especially those with hard to control eczema and/or MRSA (Methicillin resistant Staphylococcus aureus) infections.	topic_mrs
76501	4	355616	11	NULL	NULL	0	NULL	MRSA infection	Process		is a type of 					recurrent skin infections	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Dilute bleach baths have long been recommended to help children with recurrent skin infections, especially those with hard to control eczema and/or MRSA (Methicillin resistant Staphylococcus aureus) infections.	topic_mrs
76502	5	355616	11	NULL	NULL	0	NULL	eczema	MedicalFinding		treats by 					Dilute bleach baths	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Dilute bleach baths have long been recommended to help children with recurrent skin infections, especially those with hard to control eczema and/or MRSA (Methicillin resistant Staphylococcus aureus) infections.	topic_mrs
76503	6	355616	11	NULL	NULL	0	NULL	MRSA infection	Process		treats by 					Dilute bleach baths	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Dilute bleach baths have long been recommended to help children with recurrent skin infections, especially those with hard to control eczema and/or MRSA (Methicillin resistant Staphylococcus aureus) infections.	topic_mrs
75616	1	355618	11	NULL	NULL	0	NULL	Pleural empyema	MedicalFinding		also known as					pyothorax	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Pleural empyema (also known as a pyothorax or purulent pleuritis) is an accumulation of pus in the pleural cavity. Most pleural empyemas arise from an infection within the lung (pneumonia), often associated with parapneumonic effusions	topic_mrs
75617	2	355618	11	NULL	NULL	0	NULL	Pleural empyema	MedicalFinding		also known as					purulent pleuritis	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Pleural empyema (also known as a pyothorax or purulent pleuritis) is an accumulation of pus in the pleural cavity. Most pleural empyemas arise from an infection within the lung (pneumonia), often associated with parapneumonic effusions	topic_mrs
75618	3	355618	11	NULL	NULL	0	NULL	Pleural empyema	MedicalFinding		accumulates					pus	CellComponent	pleural cavity			NULL		0	NULL	NULL	NULL	NULL	NULL	Pleural empyema (also known as a pyothorax or purulent pleuritis) is an accumulation of pus in the pleural cavity. Most pleural empyemas arise from an infection within the lung (pneumonia), often associated with parapneumonic effusions	topic_mrs
75619	4	355618	11	NULL	NULL	0	NULL	pleural empyemas	MedicalFinding		arise from					pneumonia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Pleural empyema (also known as a pyothorax or purulent pleuritis) is an accumulation of pus in the pleural cavity. Most pleural empyemas arise from an infection within the lung (pneumonia), often associated with parapneumonic effusions	topic_mrs
75620	5	355618	11	NULL	NULL	0	NULL	pneumonia	MedicalFinding		infects					lung 	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Pleural empyema (also known as a pyothorax or purulent pleuritis) is an accumulation of pus in the pleural cavity. Most pleural empyemas arise from an infection within the lung (pneumonia), often associated with parapneumonic effusions	topic_mrs
75621	6	355618	11	NULL	NULL	0	NULL	Pleural empyema	MedicalFinding		associates with		may			parapneumonic effusions	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Pleural empyema (also known as a pyothorax or purulent pleuritis) is an accumulation of pus in the pleural cavity. Most pleural empyemas arise from an infection within the lung (pneumonia), often associated with parapneumonic effusions	topic_mrs
77239	1	355620	11	NULL	NULL	0	NULL	fluids	Chemical		is withdrawn from		systematically			wound	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Drainage is the systematic withdrawal of fluids and discharges from a wound, sore, or cavity.	topic_mrs
77240	2	355620	11	NULL	NULL	0	NULL	statement 1	MedicalFinding		is known as					drainage	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Drainage is the systematic withdrawal of fluids and discharges from a wound, sore, or cavity.	topic_mrs
77241	3	355620	11	NULL	NULL	0	NULL	fluids	Chemical		is withdrawn from		systematically			sore	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Drainage is the systematic withdrawal of fluids and discharges from a wound, sore, or cavity.	topic_mrs
77242	4	355620	11	NULL	NULL	0	NULL	statement 3	MedicalProcedure		is known as					drainage	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Drainage is the systematic withdrawal of fluids and discharges from a wound, sore, or cavity.	topic_mrs
77243	5	355620	11	NULL	NULL	0	NULL	fluids	Chemical		is withdrawn from		systematically			cavity	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Drainage is the systematic withdrawal of fluids and discharges from a wound, sore, or cavity.	topic_mrs
77244	6	355620	11	NULL	NULL	0	NULL	statement 5	MedicalProcedure		is known as					drainage	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Drainage is the systematic withdrawal of fluids and discharges from a wound, sore, or cavity.	topic_mrs
77245	7	355620	11	NULL	NULL	0	NULL	discharge	Chemical		is withdrawn from		systematically\t			wound	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Drainage is the systematic withdrawal of fluids and discharges from a wound, sore, or cavity.	topic_mrs
77246	8	355620	11	NULL	NULL	NULL	NULL	statement 7	MedicalFinding		is known as					drainage	MedicalProcedure				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Drainage is the systematic withdrawal of fluids and discharges from a wound, sore, or cavity.	topic_mrs
77247	9	355620	11	NULL	NULL	0	NULL	discharge	Chemical		is withdrawn from		systematically			sore	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Drainage is the systematic withdrawal of fluids and discharges from a wound, sore, or cavity.	topic_mrs
77248	10	355620	11	NULL	NULL	0	NULL	statement 9	MedicalProcedure\t		is known as					drainage	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Drainage is the systematic withdrawal of fluids and discharges from a wound, sore, or cavity.	topic_mrs
77249	11	355620	11	NULL	NULL	0	NULL	discharge	Chemical		is withdrawn from		systematically			cavity	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Drainage is the systematic withdrawal of fluids and discharges from a wound, sore, or cavity.	topic_mrs
77250	12	355620	11	NULL	NULL	0	NULL	statement 11	MedicalProcedure		is known as					drainage	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Drainage is the systematic withdrawal of fluids and discharges from a wound, sore, or cavity.	topic_mrs
76504	1	355621	11	NULL	NULL	0	NULL	MRSA pneumonia	MedicalFinding		treats by 					antimicrobial therapy	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with MRSA pneumonia complicated by empyema, antimicrobial therapy against MRSA should be used in conjunction with drainage procedures	topic_mrs
75622	1	355623	11	NULL	NULL	0	NULL	Trimethoprim-sulfamethoxazole	Chemical		is a synonym of					Co-trimoxazole	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Trimethoprim-sulfamethoxazole or Co-trimoxazole (abbreviated SXT, TMP-SMX, TMP-SMZ or TMP-sulfa) is a sulfonamide antibiotic combination of trimethoprim and sulfamethoxazole, in the ratio of 1 to 5, used in the treatment of a variety of bacterial infections. 	topic_mrs
75623	2	355623	11	NULL	NULL	0	NULL	Trimethoprim-sulfamethoxazole	Chemical		is					SXT	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Trimethoprim-sulfamethoxazole or Co-trimoxazole (abbreviated SXT, TMP-SMX, TMP-SMZ or TMP-sulfa) is a sulfonamide antibiotic combination of trimethoprim and sulfamethoxazole, in the ratio of 1 to 5, used in the treatment of a variety of bacterial infections. 	topic_mrs
75624	3	355623	11	NULL	NULL	0	NULL	Trimethoprim-sulfamethoxazole	Chemical		is					TMP-SMX	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Trimethoprim-sulfamethoxazole or Co-trimoxazole (abbreviated SXT, TMP-SMX, TMP-SMZ or TMP-sulfa) is a sulfonamide antibiotic combination of trimethoprim and sulfamethoxazole, in the ratio of 1 to 5, used in the treatment of a variety of bacterial infections. 	topic_mrs
75625	4	355623	11	NULL	NULL	0	NULL	Trimethoprim-sulfamethoxazole	Chemical		is					TMP-SMZ	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Trimethoprim-sulfamethoxazole or Co-trimoxazole (abbreviated SXT, TMP-SMX, TMP-SMZ or TMP-sulfa) is a sulfonamide antibiotic combination of trimethoprim and sulfamethoxazole, in the ratio of 1 to 5, used in the treatment of a variety of bacterial infections. 	topic_mrs
75626	5	355623	11	NULL	NULL	0	NULL	Trimethoprim-sulfamethoxazole	Chemical		is					TMP-sulfa	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Trimethoprim-sulfamethoxazole or Co-trimoxazole (abbreviated SXT, TMP-SMX, TMP-SMZ or TMP-sulfa) is a sulfonamide antibiotic combination of trimethoprim and sulfamethoxazole, in the ratio of 1 to 5, used in the treatment of a variety of bacterial infections. 	topic_mrs
75627	6	355623	11	NULL	NULL	0	NULL	Trimethoprim-sulfamethoxazole	Chemical		is a type of 					 sulfonamide antibiotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Trimethoprim-sulfamethoxazole or Co-trimoxazole (abbreviated SXT, TMP-SMX, TMP-SMZ or TMP-sulfa) is a sulfonamide antibiotic combination of trimethoprim and sulfamethoxazole, in the ratio of 1 to 5, used in the treatment of a variety of bacterial infections. 	topic_mrs
75628	7	355623	11	NULL	NULL	0	NULL	Trimethoprim-sulfamethoxazole	Chemical		treats					bacterial infections	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Trimethoprim-sulfamethoxazole or Co-trimoxazole (abbreviated SXT, TMP-SMX, TMP-SMZ or TMP-sulfa) is a sulfonamide antibiotic combination of trimethoprim and sulfamethoxazole, in the ratio of 1 to 5, used in the treatment of a variety of bacterial infections. 	topic_mrs
76514	1	355624	11	NULL	NULL	0	NULL	TMP-SMX	Chemical		is a type of 					antibiotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Some antibiotic options with parenteral and oral routes of administration include the following: TMP-SMX 4 mg/kg/dose (TMP component) twice daily	topic_mrs
76505	1	355625	11	NULL	NULL	0	NULL	Magnetic resonance imaging	Process		is a type of 					medical imaging technique	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic resonance imaging (MRI), nuclear magnetic resonance imaging (NMRI), or magnetic resonance tomography (MRT) is a medical imaging technique used in radiology to visualize detailed internal structures. 	topic_mrs
76506	2	355625	11	NULL	NULL	0	NULL	nuclear magnetic resonance imaging	Process		is a type of 					 medical imaging technique	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic resonance imaging (MRI), nuclear magnetic resonance imaging (NMRI), or magnetic resonance tomography (MRT) is a medical imaging technique used in radiology to visualize detailed internal structures. 	topic_mrs
76507	3	355625	11	NULL	NULL	0	NULL	magnetic resonance tomography	Process		is a type of 					medical imaging technique	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic resonance imaging (MRI), nuclear magnetic resonance imaging (NMRI), or magnetic resonance tomography (MRT) is a medical imaging technique used in radiology to visualize detailed internal structures. 	topic_mrs
76508	4	355625	11	NULL	NULL	0	NULL	Magnetic resonance imaging	Process		is					MRI	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic resonance imaging (MRI), nuclear magnetic resonance imaging (NMRI), or magnetic resonance tomography (MRT) is a medical imaging technique used in radiology to visualize detailed internal structures. 	topic_mrs
76509	5	355625	11	NULL	NULL	0	NULL	nuclear magnetic resonance imaging	Process		is					NMRI	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic resonance imaging (MRI), nuclear magnetic resonance imaging (NMRI), or magnetic resonance tomography (MRT) is a medical imaging technique used in radiology to visualize detailed internal structures. 	topic_mrs
76510	6	355625	11	NULL	NULL	0	NULL	magnetic resonance tomography	Process		is					MRT	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic resonance imaging (MRI), nuclear magnetic resonance imaging (NMRI), or magnetic resonance tomography (MRT) is a medical imaging technique used in radiology to visualize detailed internal structures. 	topic_mrs
76511	1	355626	11	NULL	NULL	0	NULL	Magnetic resonance imaging	Process		is					MRI	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 Magnetic resonance imaging (MRI) with gadolinium is the imaging modality of choice, particularly for detection of early osteomyelitis and associated soft-tissue diseas	topic_mrs
76512	2	355626	11	NULL	NULL	0	NULL	Magnetic resonance imaging	Process		detects					osteomyelitis	MedicalFinding	early			NULL		0	NULL	NULL	NULL	NULL	NULL	 Magnetic resonance imaging (MRI) with gadolinium is the imaging modality of choice, particularly for detection of early osteomyelitis and associated soft-tissue diseas	topic_mrs
76513	3	355626	11	NULL	NULL	0	NULL	Magnetic resonance imaging	Process		detects					soft-tissue diseas	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	 Magnetic resonance imaging (MRI) with gadolinium is the imaging modality of choice, particularly for detection of early osteomyelitis and associated soft-tissue diseas	topic_mrs
76515	1	355628	11	NULL	NULL	0	NULL	linezolid	Chemical		is an alternative to 					IV vancomycin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	IV vancomycin for 2 weeks is recommended. Alternatives include the following: linezolid 600 mg PO/IV twice daily or TMP-SMX 5 mg/kg/dose IV every 8–12 h	topic_mrs
76516	2	355628	11	NULL	NULL	0	NULL	TMP-SMX	Chemical		is an alternative to 					IV vancomycin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	IV vancomycin for 2 weeks is recommended. Alternatives include the following: linezolid 600 mg PO/IV twice daily or TMP-SMX 5 mg/kg/dose IV every 8–12 h	topic_mrs
76517	1	355629	11	NULL	NULL	0	NULL	Vancomycin	Chemical		administered in		slowly			 dilute solution	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Vancomycin must be administered in a dilute solution slowly, over at least 60 minutes (maximum rate of 10 mg/minute for doses >500 mg). This is due to the high incidence of pain and thrombophlebitis and to avoid an infusion reaction known as the red man syndrome or red neck syndrome.	topic_mrs
76518	2	355629	11	NULL	NULL	0	NULL	statement 1	Process		avoid					pain	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Vancomycin must be administered in a dilute solution slowly, over at least 60 minutes (maximum rate of 10 mg/minute for doses >500 mg). This is due to the high incidence of pain and thrombophlebitis and to avoid an infusion reaction known as the red man syndrome or red neck syndrome.	topic_mrs
76519	3	355629	11	NULL	NULL	0	NULL	statement 1	Process		avoid					thrombophlebitis	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Vancomycin must be administered in a dilute solution slowly, over at least 60 minutes (maximum rate of 10 mg/minute for doses >500 mg). This is due to the high incidence of pain and thrombophlebitis and to avoid an infusion reaction known as the red man syndrome or red neck syndrome.	topic_mrs
76520	4	355629	11	NULL	NULL	0	NULL	statement 1	Process		avoid					red man syndrome	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Vancomycin must be administered in a dilute solution slowly, over at least 60 minutes (maximum rate of 10 mg/minute for doses >500 mg). This is due to the high incidence of pain and thrombophlebitis and to avoid an infusion reaction known as the red man syndrome or red neck syndrome.	topic_mrs
76521	5	355629	11	NULL	NULL	NULL	NULL	red man syndrome	MedicalFinding		is also known as					red neck syndrome	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Vancomycin must be administered in a dilute solution slowly, over at least 60 minutes (maximum rate of 10 mg/minute for doses >500 mg). This is due to the high incidence of pain and thrombophlebitis and to avoid an infusion reaction known as the red man syndrome or red neck syndrome.	topic_mrs
76522	6	355629	11	NULL	NULL	NULL	NULL	red man syndrome	MedicalFinding		is a type of 					infusion reaction	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Vancomycin must be administered in a dilute solution slowly, over at least 60 minutes (maximum rate of 10 mg/minute for doses >500 mg). This is due to the high incidence of pain and thrombophlebitis and to avoid an infusion reaction known as the red man syndrome or red neck syndrome.	topic_mrs
76523	1	355630	11	NULL	NULL	0	NULL	osteomyelitis	MedicalFinding		is a type of 					CA-MRSA infections	Process	invasive susceptible			NULL		0	NULL	NULL	NULL	NULL	NULL	Although not speciﬁcally approved for treatment of MRSA infection, it has become widely used for treatment of SSTI and has been successfully used for treatment of invasive susceptible CA-MRSA infections in children, including osteomyelitis, septic arthritis, pneumonia, and lymphadenitis	topic_mrs
76524	2	355630	11	NULL	NULL	0	NULL	septic arthritis	MedicalFinding		is a type of 					CA-MRSA infections	Process	invasive susceptible			NULL		0	NULL	NULL	NULL	NULL	NULL	Although not speciﬁcally approved for treatment of MRSA infection, it has become widely used for treatment of SSTI and has been successfully used for treatment of invasive susceptible CA-MRSA infections in children, including osteomyelitis, septic arthritis, pneumonia, and lymphadenitis	topic_mrs
76525	3	355630	11	NULL	NULL	0	NULL	 pneumonia	MedicalFinding		is a type of 					CA-MRSA infections	Process	invasive susceptible			NULL		0	NULL	NULL	NULL	NULL	NULL	Although not speciﬁcally approved for treatment of MRSA infection, it has become widely used for treatment of SSTI and has been successfully used for treatment of invasive susceptible CA-MRSA infections in children, including osteomyelitis, septic arthritis, pneumonia, and lymphadenitis	topic_mrs
76526	4	355630	11	NULL	NULL	0	NULL	 lymphadenitis	MedicalFinding		is a type of 					CA-MRSA infection	Process	invasive susceptible			NULL		0	NULL	NULL	NULL	NULL	NULL	Although not speciﬁcally approved for treatment of MRSA infection, it has become widely used for treatment of SSTI and has been successfully used for treatment of invasive susceptible CA-MRSA infections in children, including osteomyelitis, septic arthritis, pneumonia, and lymphadenitis	topic_mrs
76527	1	355631	11	NULL	NULL	NULL	NULL	infective endocarditis	MedicalFinding		is a type of 					 endovascular infections	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because it is bacteriostatic, it is not recommended for endovascular infections, such as infective endocarditis or septic thrombophlebitis.	topic_mrs
76528	2	355631	11	NULL	NULL	NULL	NULL	 septic thrombophlebitis	MedicalFinding		is a type of 					endovascular infections	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because it is bacteriostatic, it is not recommended for endovascular infections, such as infective endocarditis or septic thrombophlebitis.	topic_mrs
75499	1	355632	5	NULL	NULL	0	NULL	MALT lymphoma patients	GroupOfPeople		infected with					H pylori	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	It has been seen that in those patients with MALT lymphoma who also test positive for H pylori, antibiotics for H pylori may actually control the cancer.	topic_ll
75500	2	355632	5	NULL	NULL	0	NULL	H pylori antibiotics	Chemical		control					MALT lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	It has been seen that in those patients with MALT lymphoma who also test positive for H pylori, antibiotics for H pylori may actually control the cancer.	topic_ll
75501	1	355633	5	NULL	NULL	0	NULL	MALT lymphoma	MedicalFinding		affects		most commonly			stomach	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	The most commonly affected organ is the stomach, which accounts for nearly 2 out of every 3 cases. But other organs are also affected by MALT lymphoma.	topic_ll
75502	1	355634	5	NULL	NULL	0	NULL	MALT lymphoma	MedicalFinding		affects					stomach	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	The symptoms of MALT lymphoma depend on the organ affected. When MALT lymphoma affects the stomach, you may feel indigestion, weight loss and black stools because of bleeding into the stomach. Some people may feel a vague pain in the abdomen.	topic_ll
75503	2	355634	5	NULL	NULL	0	NULL	indigestion	MedicalFinding		is a symptom of					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The symptoms of MALT lymphoma depend on the organ affected. When MALT lymphoma affects the stomach, you may feel indigestion, weight loss and black stools because of bleeding into the stomach. Some people may feel a vague pain in the abdomen.	topic_ll
75504	3	355634	5	NULL	NULL	0	NULL	weight loss	MedicalFinding		is a symptom of					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The symptoms of MALT lymphoma depend on the organ affected. When MALT lymphoma affects the stomach, you may feel indigestion, weight loss and black stools because of bleeding into the stomach. Some people may feel a vague pain in the abdomen.	topic_ll
75505	4	355634	5	NULL	NULL	0	NULL	black stools	MedicalFinding		is a symptom of					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The symptoms of MALT lymphoma depend on the organ affected. When MALT lymphoma affects the stomach, you may feel indigestion, weight loss and black stools because of bleeding into the stomach. Some people may feel a vague pain in the abdomen.	topic_ll
75506	5	355634	5	NULL	NULL	0	NULL	stomach	OrganismPart	bleeding of	causes					black stools	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The symptoms of MALT lymphoma depend on the organ affected. When MALT lymphoma affects the stomach, you may feel indigestion, weight loss and black stools because of bleeding into the stomach. Some people may feel a vague pain in the abdomen.	topic_ll
75507	6	355634	5	NULL	NULL	0	NULL	abdominal pain	MedicalFinding	vague	is a symptom of					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The symptoms of MALT lymphoma depend on the organ affected. When MALT lymphoma affects the stomach, you may feel indigestion, weight loss and black stools because of bleeding into the stomach. Some people may feel a vague pain in the abdomen.	topic_ll
75963	1	355635	11	NULL	NULL	0	NULL	Beta-lactamase	GP		is					enzyme	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Beta-lactamases are enzymes produced by some bacteria and are responsible for their resistance to beta-lactam antibiotics like penicillins, cephamycins, and carbapenems (ertapenem).	topic_mrs
75964	2	355635	11	NULL	NULL	0	NULL	Beta-lactamases	GP		produced by					bacteria	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Beta-lactamases are enzymes produced by some bacteria and are responsible for their resistance to beta-lactam antibiotics like penicillins, cephamycins, and carbapenems (ertapenem).	topic_mrs
75965	3	355635	11	NULL	NULL	0	NULL	penicillins	Chemical		is a type of 					beta-lactam antibiotics	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Beta-lactamases are enzymes produced by some bacteria and are responsible for their resistance to beta-lactam antibiotics like penicillins, cephamycins, and carbapenems (ertapenem).	topic_mrs
75966	4	355635	11	NULL	NULL	0	NULL	cephamycins	Chemical		is a type of 					beta-lactam antibiotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Beta-lactamases are enzymes produced by some bacteria and are responsible for their resistance to beta-lactam antibiotics like penicillins, cephamycins, and carbapenems (ertapenem).	topic_mrs
75967	5	355635	11	NULL	NULL	0	NULL	carbapenems	Chemical		is a type of 					beta-lactam antibiotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Beta-lactamases are enzymes produced by some bacteria and are responsible for their resistance to beta-lactam antibiotics like penicillins, cephamycins, and carbapenems (ertapenem).	topic_mrs
75968	6	355635	11	NULL	NULL	0	NULL	carbapenems	Chemical		is a synonym of					ertapenem	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Beta-lactamases are enzymes produced by some bacteria and are responsible for their resistance to beta-lactam antibiotics like penicillins, cephamycins, and carbapenems (ertapenem).	topic_mrs
75508	1	355636	5	NULL	NULL	0	NULL	follicular lymphoma	MedicalFinding	risk of	is associated with		possibly			diet	Food				NULL		0	NULL	NULL	NULL	NULL	NULL	Studies suggest risk of follicular lymphoma is associated with a person's diet to say the least.  A new study linked nitrite intake with increased risk of follicular lymphoma.	topic_ll
75509	2	355636	5	NULL	NULL	0	NULL	nitrite	Chemical	intake of	increases					follicular lymphoma	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	Studies suggest risk of follicular lymphoma is associated with a person's diet to say the least.  A new study linked nitrite intake with increased risk of follicular lymphoma.	topic_ll
76129	1	355638	11	NULL	NULL	0	NULL	Bacteremia	MedicalFinding		is the presence of					bacteria	Organism	in the blood			NULL		0	NULL	NULL	NULL	NULL	NULL	Bacteremia (also Bacteraemia or Bacteræmia) is the presence of bacteria in the blood. The blood is normally a sterile environment, so the detection of bacteria in the blood (most commonly with blood cultures) is always abnormal.	topic_mrs
76130	2	355638	11	NULL	NULL	0	NULL	Bacteremia	MedicalFinding		is a synonym of					Bacteraemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Bacteremia (also Bacteraemia or Bacteræmia) is the presence of bacteria in the blood. The blood is normally a sterile environment, so the detection of bacteria in the blood (most commonly with blood cultures) is always abnormal.	topic_mrs
76131	3	355638	11	NULL	NULL	0	NULL	 blood	OrganismPart		is		normally			sterile	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Bacteremia (also Bacteraemia or Bacteræmia) is the presence of bacteria in the blood. The blood is normally a sterile environment, so the detection of bacteria in the blood (most commonly with blood cultures) is always abnormal.	topic_mrs
76166	4	355638	11	NULL	NULL	0	NULL	Bacteremia	MedicalFinding		is always					abnormal	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Bacteremia (also Bacteraemia or Bacteræmia) is the presence of bacteria in the blood. The blood is normally a sterile environment, so the detection of bacteria in the blood (most commonly with blood cultures) is always abnormal.	topic_mrs
75953	1	355639	5	NULL	NULL	0	NULL	Resveratrol	Chemical		induces					apoptosis	process				NULL	OCI-LY8 cells	0	NULL	NULL	NULL	NULL	NULL	Resveratrol induces apoptosis in transformed follicular lymphoma OCI-LY8 cells: Evidence for a novel mechanism involving inhibition of BCL6 signaling	topic_ll
75954	2	355639	5	NULL	NULL	0	NULL	OCI-LY8	Cell		is a type of					transformed follicular lymphoma cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Resveratrol induces apoptosis in transformed follicular lymphoma OCI-LY8 cells: Evidence for a novel mechanism involving inhibition of BCL6 signaling	topic_ll
75955	3	355639	5	NULL	NULL	0	NULL	statement 1	Process		inhibits					BCL6 signaling	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Resveratrol induces apoptosis in transformed follicular lymphoma OCI-LY8 cells: Evidence for a novel mechanism involving inhibition of BCL6 signaling	topic_ll
76529	1	355641	11	NULL	NULL	NULL	NULL	echocardiogram	MedicalProcedure		is also known as					 cardiac ECHO 	MedicalProcedure				NULL		NULL	NULL	NULL	NULL	NULL	NULL	An echocardiogram, often referred to in the medical community as a cardiac ECHO or simply an ECHO, is a sonogram of the heart...an echocardiogram can also produce accurate assessment of the velocity of blood and cardiac tissue	topic_mrs
76530	2	355641	11	NULL	NULL	NULL	NULL	echocardiogram	MedicalProcedure		is also known as					ECHO	MedicalProcedure				NULL		NULL	NULL	NULL	NULL	NULL	NULL	An echocardiogram, often referred to in the medical community as a cardiac ECHO or simply an ECHO, is a sonogram of the heart...an echocardiogram can also produce accurate assessment of the velocity of blood and cardiac tissue	topic_mrs
76531	3	355641	11	NULL	NULL	NULL	NULL	 echocardiogram	MedicalProcedure		is a type of 					sonogram	MedicalProcedure	heart			NULL		NULL	NULL	NULL	NULL	NULL	NULL	An echocardiogram, often referred to in the medical community as a cardiac ECHO or simply an ECHO, is a sonogram of the heart...an echocardiogram can also produce accurate assessment of the velocity of blood and cardiac tissue	topic_mrs
76532	4	355641	11	NULL	NULL	NULL	NULL	echocardiogram	MedicalProcedure		 assess 					blood	OrganismPart	velocity of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	An echocardiogram, often referred to in the medical community as a cardiac ECHO or simply an ECHO, is a sonogram of the heart...an echocardiogram can also produce accurate assessment of the velocity of blood and cardiac tissue	topic_mrs
76533	5	355641	11	NULL	NULL	0	NULL	echocardiogram	MedicalProcedure		assess					cardiac tissue	Organism part				NULL		0	NULL	NULL	NULL	NULL	NULL	An echocardiogram, often referred to in the medical community as a cardiac ECHO or simply an ECHO, is a sonogram of the heart...an echocardiogram can also produce accurate assessment of the velocity of blood and cardiac tissue	topic_mrs
75956	1	355642	5	NULL	NULL	0	NULL	dust	Chemical	exposure to	is not linked to					cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	As if being involved in the 9/11 attack on the World Trade Centers wasn't horrific enough, it's now appearing as if people present at the WTC on that world-changing day have higher than normal rates of lymphatic and blood cancers. While New York city's health commissioner has said there is no evidence linking dust exposure to cancer, the Medical Monitoring Program reports a "handful of cases of multiple myeloma in very young individuals." They add, "multiple myeloma is a condition that ... almost aways presents later in life." NULL	topic_ll
76172	1	355643	11	NULL	NULL	0	NULL	Echocardiography	MedicalProcedure		is recommended for					bacteremia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Echocardiography is recommended for all adult patients with bacteremia	topic_mrs
75957	1	355644	5	NULL	NULL	0	NULL	uranium miners	GroupOfPeople		prone to					leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Leukemia among uranium miners--late effects of exposure to uranium dust?	topic_ll
75958	1	355645	5	NULL	NULL	0	NULL	miners	GroupOfPeople	underground	is at risk of					leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Radon and leukemia risk in underground miners: are working level months the most appropriate exposure parameter?	topic_ll
75959	2	355645	5	NULL	NULL	0	NULL	radon	Chemical		plays a role in		possibly			statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Radon and leukemia risk in underground miners: are working level months the most appropriate exposure parameter?	topic_ll
76174	1	355646	11	NULL	NULL	0	NULL	Daptomycin	Chemical		is a type of 					lipopeptide class antibiotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Daptomycin is a lipopeptide class antibiotic that disrupts cell membrane function via calcium-dependent binding, resulting in bactericidal activity in a concentration-dependent fashion	topic_mrs
76176	2	355646	11	NULL	NULL	0	NULL	Daptomycin	Chemical		disrupts					cell membrane	CellComponent				NULL		0	NULL	NULL	NULL	NULL	NULL	Daptomycin is a lipopeptide class antibiotic that disrupts cell membrane function via calcium-dependent binding, resulting in bactericidal activity in a concentration-dependent fashion	topic_mrs
76178	3	355646	11	NULL	NULL	0	NULL	calcium-dependent binding	Process		disrupts in 					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Daptomycin is a lipopeptide class antibiotic that disrupts cell membrane function via calcium-dependent binding, resulting in bactericidal activity in a concentration-dependent fashion	topic_mrs
76179	4	355646	11	NULL	NULL	0	NULL	statement 2	Process		resulted in					 bactericidal activity	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Daptomycin is a lipopeptide class antibiotic that disrupts cell membrane function via calcium-dependent binding, resulting in bactericidal activity in a concentration-dependent fashion	topic_mrs
76181	5	355646	11	NULL	NULL	0	NULL	statement 4	Process		is in a					concentration-dependent fashion	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Daptomycin is a lipopeptide class antibiotic that disrupts cell membrane function via calcium-dependent binding, resulting in bactericidal activity in a concentration-dependent fashion	topic_mrs
76184	1	355647	11	NULL	NULL	0	NULL	Daptomycin	Chemical		not treat					non-hematogenous MRSA pneumonia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Daptomycin should not be used for the treatment of non-hematogenous MRSA pneumonia, because its activity is inhibited by pulmonary surfactant.	topic_mrs
76185	2	355647	11	NULL	NULL	0	NULL	Daptomycin	Chemical		inhibited by					pulmonary surfactant	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Daptomycin should not be used for the treatment of non-hematogenous MRSA pneumonia, because its activity is inhibited by pulmonary surfactant.	topic_mrs
76192	1	355650	11	NULL	NULL	0	NULL	vancomycin 	Chemical		 cross-resist with		possibly			daptomycin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Prior exposure to vancomycin and elevated vancomycin MICs have been associated with increases in daptomycin MICs, suggesting possible cross-resistance	topic_mrs
76201	1	355651	11	NULL	NULL	0	NULL	Quinupristin	Chemical		is a type of 					streptogramin antibiotics	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Quinupristin-dalfopristin is a combination of 2 streptogramin antibiotics and inhibits protein synthesis	topic_mrs
76202	2	355651	11	NULL	NULL	0	NULL	dalfopristin	Chemical		is a type of 					streptogramin antibiotics	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Quinupristin-dalfopristin is a combination of 2 streptogramin antibiotics and inhibits protein synthesis	topic_mrs
76204	3	355651	11	NULL	NULL	0	NULL	Quinupristin	Chemical		combines with					dalfopristin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Quinupristin-dalfopristin is a combination of 2 streptogramin antibiotics and inhibits protein synthesis	topic_mrs
76206	4	355651	11	NULL	NULL	0	NULL	statement 3	Process		inhibits					protein synthesis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Quinupristin-dalfopristin is a combination of 2 streptogramin antibiotics and inhibits protein synthesis	topic_mrs
76209	1	355653	11	NULL	NULL	0	NULL	Quinupristin-Dalfopristin	Chemical		is approved for		 FDA			cSSTI	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Quinupristin-Dalfopristin  is FDA-approved for cSSTI in adults and children greater than 16 years of age.	topic_mrs
76212	1	355654	11	NULL	NULL	0	NULL	Rifampin	Chemical		has					bactericidal activity	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Rifampin has bactericidal activity against S. aureus and achieves high intracellular levels, in addition to penetrating bioﬁlms	topic_mrs
76213	2	355654	11	NULL	NULL	0	NULL	statement 1	Process		is against					S. aureus	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Rifampin has bactericidal activity against S. aureus and achieves high intracellular levels, in addition to penetrating bioﬁlms	topic_mrs
76214	3	355654	11	NULL	NULL	0	NULL	Rifampin	Chemical		 achieves					high intracellular levels	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Rifampin has bactericidal activity against S. aureus and achieves high intracellular levels, in addition to penetrating bioﬁlms	topic_mrs
76215	4	355654	11	NULL	NULL	0	NULL	Rifampin	Chemical		penetrate					biofilms	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Rifampin has bactericidal activity against S. aureus and achieves high intracellular levels, in addition to penetrating bioﬁlms	topic_mrs
76216	1	355655	11	NULL	NULL	0	NULL	biofilm	Organism		is an aggregate of					microorganisms	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	A biofilm is an aggregate of microorganisms in which cells adhere to each other and/or to a surface. These adherent cells are frequently embedded within a self-produced matrix of extracellular polymeric substance (EPS)	topic_mrs
76217	2	355655	11	NULL	NULL	0	NULL	statement 1	Process		are embedded within		frequently			extracellular polymeric substance	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	A biofilm is an aggregate of microorganisms in which cells adhere to each other and/or to a surface. These adherent cells are frequently embedded within a self-produced matrix of extracellular polymeric substance (EPS)	topic_mrs
76218	3	355655	11	NULL	NULL	0	NULL	extracellular polymeric substance	Chemical		is					EPS	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	A biofilm is an aggregate of microorganisms in which cells adhere to each other and/or to a surface. These adherent cells are frequently embedded within a self-produced matrix of extracellular polymeric substance (EPS)	topic_mrs
76219	4	355655	11	NULL	NULL	0	NULL	extracellular polymeric substance	Chemical		is a product of					biofilm	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	A biofilm is an aggregate of microorganisms in which cells adhere to each other and/or to a surface. These adherent cells are frequently embedded within a self-produced matrix of extracellular polymeric substance (EPS)	topic_mrs
76220	1	355656	11	NULL	NULL	0	NULL	 biofilm	Organism		is held together by					 EPS	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The biofilm is held together and protected by a matrix of excreted polymeric compounds called EPS. EPS is an abbreviation for either extracellular polymeric substance or exopolysaccharide. This matrix protects the cells within it and facilitates communication among them through biochemical signals.	topic_mrs
76221	2	355656	11	NULL	NULL	0	NULL	 EPS	Chemical		is					extracellular polymeric substance	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The biofilm is held together and protected by a matrix of excreted polymeric compounds called EPS. EPS is an abbreviation for either extracellular polymeric substance or exopolysaccharide. This matrix protects the cells within it and facilitates communication among them through biochemical signals.	topic_mrs
76222	3	355656	11	NULL	NULL	0	NULL	EPS	Chemical		is a type of 					exopolysaccharide	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The biofilm is held together and protected by a matrix of excreted polymeric compounds called EPS. EPS is an abbreviation for either extracellular polymeric substance or exopolysaccharide. This matrix protects the cells within it and facilitates communication among them through biochemical signals.	topic_mrs
76223	4	355656	11	NULL	NULL	0	NULL	EPS	Chemical		protects					cells	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	The biofilm is held together and protected by a matrix of excreted polymeric compounds called EPS. EPS is an abbreviation for either extracellular polymeric substance or exopolysaccharide. This matrix protects the cells within it and facilitates communication among them through biochemical signals.	topic_mrs
76224	5	355656	11	NULL	NULL	0	NULL	EPS	Chemical		facilitates					communication	Process	 by biochemical signals			NULL		0	NULL	NULL	NULL	NULL	NULL	The biofilm is held together and protected by a matrix of excreted polymeric compounds called EPS. EPS is an abbreviation for either extracellular polymeric substance or exopolysaccharide. This matrix protects the cells within it and facilitates communication among them through biochemical signals.	topic_mrs
76227	1	355657	7	NULL	NULL	NULL	NULL	methylation	Process		crucial role in					polyp/adenoma	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings suggest a potentially crucial role for methylation in the polyp/adenoma to cancer progression in colorectal carcinogenesis	topic_ccc
76228	2	355657	7	NULL	NULL	NULL	NULL	polyp/adenoma	MedicalFinding		progressed to					cancer	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings suggest a potentially crucial role for methylation in the polyp/adenoma to cancer progression in colorectal carcinogenesis	topic_ccc
76554	3	355657	7	NULL	NULL	0	NULL	statement 2	Process		occur in					colorectal carcinogenesis	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest a potentially crucial role for methylation in the polyp/adenoma to cancer progression in colorectal carcinogenesis	topic_ccc
76534	1	355658	7	11	NULL	0	NULL	Stage 2 colon cancer	MedicalFinding		is also known as					Duke's B colon cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Stage 2 colon cancer used to be called Duke's B colon cancer.	topic_ccc
76556	1	355661	7	NULL	NULL	0	NULL	RASSF1A	GP		methylated in		frequently			 mucosae	OrganismPart	distal normal-appearing			NULL		0	NULL	NULL	NULL	NULL	NULL	Along with RASSF1A and SFRP1, two identified genes, HOXA5 and PDE10A, were also frequently methylated in distal normal-appearing mucosae and CRCs. 	topic_ccc
76557	2	355661	7	NULL	NULL	NULL	NULL	RASSF1A	GP		methylated in		frequently			CRC	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Along with RASSF1A and SFRP1, two identified genes, HOXA5 and PDE10A, were also frequently methylated in distal normal-appearing mucosae and CRCs. 	topic_ccc
76558	3	355661	7	NULL	NULL	NULL	NULL	SFRP1	GP		methylated in		frequently			mucosae 	OrganismPart	distal normal-appearing			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Along with RASSF1A and SFRP1, two identified genes, HOXA5 and PDE10A, were also frequently methylated in distal normal-appearing mucosae and CRCs. 	topic_ccc
76559	4	355661	7	NULL	NULL	NULL	NULL	SFRP1	GP		methylated in		frequently			CRC	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Along with RASSF1A and SFRP1, two identified genes, HOXA5 and PDE10A, were also frequently methylated in distal normal-appearing mucosae and CRCs. 	topic_ccc
76560	5	355661	7	NULL	NULL	0	NULL	HOXA5 	GP		methylated in		frequently			mucosae 	OrganismPart	distal normal-appearing			NULL		0	NULL	NULL	NULL	NULL	NULL	Along with RASSF1A and SFRP1, two identified genes, HOXA5 and PDE10A, were also frequently methylated in distal normal-appearing mucosae and CRCs. 	topic_ccc
76561	6	355661	7	NULL	NULL	NULL	NULL	HOXA5 	GP		methylated in		frequently			CRC	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Along with RASSF1A and SFRP1, two identified genes, HOXA5 and PDE10A, were also frequently methylated in distal normal-appearing mucosae and CRCs. 	topic_ccc
76562	7	355661	7	NULL	NULL	0	NULL	PDE10A	GP		methylated in		frequently			mucosae 	OrganismPart	distal normal-appearing			NULL		0	NULL	NULL	NULL	NULL	NULL	Along with RASSF1A and SFRP1, two identified genes, HOXA5 and PDE10A, were also frequently methylated in distal normal-appearing mucosae and CRCs. 	topic_ccc
76563	8	355661	7	NULL	NULL	0	NULL	PDE10A	GP		methylated in		frequently			CRC	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Along with RASSF1A and SFRP1, two identified genes, HOXA5 and PDE10A, were also frequently methylated in distal normal-appearing mucosae and CRCs. 	topic_ccc
76564	1	355663	7	NULL	NULL	0	NULL	A(3) receptor	GP		subtype of		abundant			cancer tissues	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	 At a protein levels low amount of A(1), A(2A), and A(2B) receptors were detected, whilst the A(3) was the most abundant subtype in both cancer tissues and cells, with a pharmacological profile typical of the A(3) subtype.	topic_ccc
76565	2	355663	7	NULL	NULL	0	NULL	A(3) receptor	GP		subtype of		abundant			cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	 At a protein levels low amount of A(1), A(2A), and A(2B) receptors were detected, whilst the A(3) was the most abundant subtype in both cancer tissues and cells, with a pharmacological profile typical of the A(3) subtype.	topic_ccc
76566	1	355664	7	NULL	NULL	0	NULL	Adenosine 	Chemical		interacts with					A(1) receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Adenosine may affect several pathophysiological processes, including cellular proliferation, through interaction with A(1), A(2A), A(2B), and A(3) receptors. In this study we characterized adenosine receptors in human colon cancer tissues and in colon cancer cell lines Caco2, DLD1, HT29. mRNA of all adenosine subtypes was detected in cancer tissues and cell lines. 	topic_ccc
76567	2	355664	7	NULL	NULL	0	NULL	Adenosine	Chemical		interacts with					A(2A) receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Adenosine may affect several pathophysiological processes, including cellular proliferation, through interaction with A(1), A(2A), A(2B), and A(3) receptors. In this study we characterized adenosine receptors in human colon cancer tissues and in colon cancer cell lines Caco2, DLD1, HT29. mRNA of all adenosine subtypes was detected in cancer tissues and cell lines. 	topic_ccc
76568	3	355664	7	NULL	NULL	0	NULL	Adenosine	Chemical		interacts with					A(2B) receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Adenosine may affect several pathophysiological processes, including cellular proliferation, through interaction with A(1), A(2A), A(2B), and A(3) receptors. In this study we characterized adenosine receptors in human colon cancer tissues and in colon cancer cell lines Caco2, DLD1, HT29. mRNA of all adenosine subtypes was detected in cancer tissues and cell lines. 	topic_ccc
76569	4	355664	7	NULL	NULL	0	NULL	Adenosine	Chemical		interacts with					A(3) receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Adenosine may affect several pathophysiological processes, including cellular proliferation, through interaction with A(1), A(2A), A(2B), and A(3) receptors. In this study we characterized adenosine receptors in human colon cancer tissues and in colon cancer cell lines Caco2, DLD1, HT29. mRNA of all adenosine subtypes was detected in cancer tissues and cell lines. 	topic_ccc
76570	5	355664	7	NULL	NULL	NULL	NULL	Adenosine	Chemical		affect		may			cellular proliferation	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Adenosine may affect several pathophysiological processes, including cellular proliferation, through interaction with A(1), A(2A), A(2B), and A(3) receptors. In this study we characterized adenosine receptors in human colon cancer tissues and in colon cancer cell lines Caco2, DLD1, HT29. mRNA of all adenosine subtypes was detected in cancer tissues and cell lines. 	topic_ccc
76571	6	355664	7	NULL	NULL	0	NULL	cellular proliferation	Process		is a type of					pathophysiological process	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Adenosine may affect several pathophysiological processes, including cellular proliferation, through interaction with A(1), A(2A), A(2B), and A(3) receptors. In this study we characterized adenosine receptors in human colon cancer tissues and in colon cancer cell lines Caco2, DLD1, HT29. mRNA of all adenosine subtypes was detected in cancer tissues and cell lines. 	topic_ccc
76572	7	355664	7	NULL	NULL	0	NULL	adenosine receptor	GP		characterized in					colon cancer tissues	OrganismPart	human			NULL		0	NULL	NULL	NULL	NULL	NULL	Adenosine may affect several pathophysiological processes, including cellular proliferation, through interaction with A(1), A(2A), A(2B), and A(3) receptors. In this study we characterized adenosine receptors in human colon cancer tissues and in colon cancer cell lines Caco2, DLD1, HT29. mRNA of all adenosine subtypes was detected in cancer tissues and cell lines. 	topic_ccc
76573	8	355664	7	NULL	NULL	0	NULL	adenosine receptor	GP		characterized in					Caco2	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Adenosine may affect several pathophysiological processes, including cellular proliferation, through interaction with A(1), A(2A), A(2B), and A(3) receptors. In this study we characterized adenosine receptors in human colon cancer tissues and in colon cancer cell lines Caco2, DLD1, HT29. mRNA of all adenosine subtypes was detected in cancer tissues and cell lines. 	topic_ccc
76574	9	355664	7	NULL	NULL	0	NULL	adenosine receptor	GP		characterized in					DLD1	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Adenosine may affect several pathophysiological processes, including cellular proliferation, through interaction with A(1), A(2A), A(2B), and A(3) receptors. In this study we characterized adenosine receptors in human colon cancer tissues and in colon cancer cell lines Caco2, DLD1, HT29. mRNA of all adenosine subtypes was detected in cancer tissues and cell lines. 	topic_ccc
76575	10	355664	7	NULL	NULL	0	NULL	adenosine receptor	GP		characterized in					HT29	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Adenosine may affect several pathophysiological processes, including cellular proliferation, through interaction with A(1), A(2A), A(2B), and A(3) receptors. In this study we characterized adenosine receptors in human colon cancer tissues and in colon cancer cell lines Caco2, DLD1, HT29. mRNA of all adenosine subtypes was detected in cancer tissues and cell lines. 	topic_ccc
76576	11	355664	7	NULL	NULL	0	NULL	Caco2	Cell		is a type of					 colon cancer cell line	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Adenosine may affect several pathophysiological processes, including cellular proliferation, through interaction with A(1), A(2A), A(2B), and A(3) receptors. In this study we characterized adenosine receptors in human colon cancer tissues and in colon cancer cell lines Caco2, DLD1, HT29. mRNA of all adenosine subtypes was detected in cancer tissues and cell lines. 	topic_ccc
76577	12	355664	7	NULL	NULL	0	NULL	DLD1	Cell		is a type of					colon cancer cell line	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Adenosine may affect several pathophysiological processes, including cellular proliferation, through interaction with A(1), A(2A), A(2B), and A(3) receptors. In this study we characterized adenosine receptors in human colon cancer tissues and in colon cancer cell lines Caco2, DLD1, HT29. mRNA of all adenosine subtypes was detected in cancer tissues and cell lines. 	topic_ccc
76578	13	355664	7	NULL	NULL	0	NULL	HT29	Cell		is a type of					colon cancer cell line	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Adenosine may affect several pathophysiological processes, including cellular proliferation, through interaction with A(1), A(2A), A(2B), and A(3) receptors. In this study we characterized adenosine receptors in human colon cancer tissues and in colon cancer cell lines Caco2, DLD1, HT29. mRNA of all adenosine subtypes was detected in cancer tissues and cell lines. 	topic_ccc
76579	1	355665	7	NULL	NULL	NULL	NULL	 sleep latency	MedicalFinding	Prolonged	polysomnographic features in 					bipolar disorder	MedicalFinding	patients with			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Prolonged sleep latency, reduced sleep efficiency, increased number and duration of awakenings, reduced delta sleep, shortened REM sleep latency, and increased REM density are common polysomnographic features in patients with bipolar disorder.	topic_bd
76580	2	355665	7	NULL	NULL	NULL	NULL	 sleep efficiency	MedicalFinding	reduced	polysomnographic features in					bipolar disorder	MedicalFinding	patients with			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Prolonged sleep latency, reduced sleep efficiency, increased number and duration of awakenings, reduced delta sleep, shortened REM sleep latency, and increased REM density are common polysomnographic features in patients with bipolar disorder.	topic_bd
76581	3	355665	7	NULL	NULL	NULL	NULL	awakenings	MedicalFinding	increased number and duration of 	polysomnographic features in					bipolar disorder	MedicalFinding	patients with			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Prolonged sleep latency, reduced sleep efficiency, increased number and duration of awakenings, reduced delta sleep, shortened REM sleep latency, and increased REM density are common polysomnographic features in patients with bipolar disorder.	topic_bd
76582	4	355665	7	NULL	NULL	NULL	NULL	delta sleep	MedicalFinding	reduced	polysomnographic features in					bipolar disorder	MedicalFinding	patients with			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Prolonged sleep latency, reduced sleep efficiency, increased number and duration of awakenings, reduced delta sleep, shortened REM sleep latency, and increased REM density are common polysomnographic features in patients with bipolar disorder.	topic_bd
76583	5	355665	7	NULL	NULL	0	NULL	REM sleep latency	MedicalFinding	shortened	polysomnographic features in					bipolar disorder	MedicalFinding	patients with			NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged sleep latency, reduced sleep efficiency, increased number and duration of awakenings, reduced delta sleep, shortened REM sleep latency, and increased REM density are common polysomnographic features in patients with bipolar disorder.	topic_bd
76584	6	355665	7	NULL	NULL	0	NULL	REM density 	MedicalFinding	increased	polysomnographic features in					bipolar disorder	MedicalFinding	patients with			NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged sleep latency, reduced sleep efficiency, increased number and duration of awakenings, reduced delta sleep, shortened REM sleep latency, and increased REM density are common polysomnographic features in patients with bipolar disorder.	topic_bd
76625	1	355666	7	NULL	NULL	NULL	NULL	S100A4 protein	GP	expression of	predictor of					colorectal cancer	MedicalFinding	recurrence in			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Expression of protein S100A4 is a predictor of recurrence in colorectal cancer.	topic_ccc
76626	1	355667	7	NULL	NULL	0	NULL	Luvox	Chemical		is a type of					antidepressant 	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Luvox - Generic Fluvoxamine - which is a prescription antidepressant of the SSRI classification that may be used in the treatment of bipolar bipolar disorder and other mental illnesses.	topic_bd
76627	2	355667	7	NULL	NULL	0	NULL	Luvox	Chemical		is used in the					bipolar disorder	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	Luvox - Generic Fluvoxamine - which is a prescription antidepressant of the SSRI classification that may be used in the treatment of bipolar bipolar disorder and other mental illnesses.	topic_bd
76628	3	355667	7	NULL	NULL	NULL	NULL	Luvox	Chemical		belongs to					SSRI 	Chemical	classification of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Luvox - Generic Fluvoxamine - which is a prescription antidepressant of the SSRI classification that may be used in the treatment of bipolar bipolar disorder and other mental illnesses.	topic_bd
76629	4	355667	7	NULL	NULL	NULL	NULL	Luvox	Chemical	generic name of	 is					Fluvoxamine	Chemical				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Luvox - Generic Fluvoxamine - which is a prescription antidepressant of the SSRI classification that may be used in the treatment of bipolar bipolar disorder and other mental illnesses.	topic_bd
76630	5	355667	7	NULL	NULL	0	NULL	Luvox	Chemical		is used in the					mental illness	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	Luvox - Generic Fluvoxamine - which is a prescription antidepressant of the SSRI classification that may be used in the treatment of bipolar bipolar disorder and other mental illnesses.	topic_bd
76631	1	355668	7	NULL	NULL	0	NULL	adenoma	MedicalFinding		distinguished from					fully blown colon carcinoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Defensin alpha 6 (DEFA 6) overexpression threshold of over 60 fold can distinguish between adenoma and fully blown colon carcinoma in individual patients.	topic_ccc
76632	2	355668	7	NULL	NULL	0	NULL	DEFA 6	GP	overexpression of	helps in					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Defensin alpha 6 (DEFA 6) overexpression threshold of over 60 fold can distinguish between adenoma and fully blown colon carcinoma in individual patients.	topic_ccc
76633	3	355668	7	NULL	NULL	0	NULL	DEFA 6	GP		is					Defensin alpha 6	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Defensin alpha 6 (DEFA 6) overexpression threshold of over 60 fold can distinguish between adenoma and fully blown colon carcinoma in individual patients.	topic_ccc
76634	1	355669	7	NULL	NULL	NULL	NULL	SSRI	Chemical		used as					antidepressant 	Chemical				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Selective serotonin reuptake inhibitors or serotonin-specific reuptake inhibitor[1] (SSRIs) are a class of compounds typically used as antidepressants in the treatment of depression, anxiety disorders, and some personality disorders.	topic_bd
76636	2	355669	7	NULL	NULL	NULL	NULL	SSRI	Chemical		used in the 					depression	MedicalFinding	treatment of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Selective serotonin reuptake inhibitors or serotonin-specific reuptake inhibitor[1] (SSRIs) are a class of compounds typically used as antidepressants in the treatment of depression, anxiety disorders, and some personality disorders.	topic_bd
76637	3	355669	7	NULL	NULL	NULL	NULL	SSRI	Chemical		used in the 					anxiety disorders	MedicalFinding	treatment of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Selective serotonin reuptake inhibitors or serotonin-specific reuptake inhibitor[1] (SSRIs) are a class of compounds typically used as antidepressants in the treatment of depression, anxiety disorders, and some personality disorders.	topic_bd
76638	4	355669	7	NULL	NULL	NULL	NULL	SSRI	Chemical		used in the					personality disorders	MedicalFinding	treatment of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Selective serotonin reuptake inhibitors or serotonin-specific reuptake inhibitor[1] (SSRIs) are a class of compounds typically used as antidepressants in the treatment of depression, anxiety disorders, and some personality disorders.	topic_bd
76642	5	355669	7	NULL	NULL	NULL	NULL	SSRI	Chemical		is					serotonin-specific reuptake inhibitor	Chemical				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Selective serotonin reuptake inhibitors or serotonin-specific reuptake inhibitor[1] (SSRIs) are a class of compounds typically used as antidepressants in the treatment of depression, anxiety disorders, and some personality disorders.	topic_bd
76643	6	355669	7	NULL	NULL	0	NULL	SSRI	Chemical		is					Selective serotonin reuptake inhibitors	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Selective serotonin reuptake inhibitors or serotonin-specific reuptake inhibitor[1] (SSRIs) are a class of compounds typically used as antidepressants in the treatment of depression, anxiety disorders, and some personality disorders.	topic_bd
76644	7	355669	7	NULL	NULL	0	NULL	statement 5	Process		is an alternative to					statement 6	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Selective serotonin reuptake inhibitors or serotonin-specific reuptake inhibitor[1] (SSRIs) are a class of compounds typically used as antidepressants in the treatment of depression, anxiety disorders, and some personality disorders.	topic_bd
76645	1	355671	7	NULL	NULL	0	NULL	SSRI	Chemical		first-line choice					bipolar disease	MedicalFinding	for the depressed phase of			NULL		0	NULL	NULL	NULL	NULL	NULL	Selective serotonin reuptake inhibitors (SSRIs) and other new antidepressants, such as buproprion and venlafaxine, are generally considered to be the first-line choices for the depressed phase of bipolar disease.	topic_bd
76646	2	355671	7	NULL	NULL	0	NULL	buproprion	Chemical		is a type of					new antidepressant	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Selective serotonin reuptake inhibitors (SSRIs) and other new antidepressants, such as buproprion and venlafaxine, are generally considered to be the first-line choices for the depressed phase of bipolar disease.	topic_bd
76647	3	355671	7	NULL	NULL	0	NULL	venlafaxine	Chemical		is a type of					new antidepressant 	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Selective serotonin reuptake inhibitors (SSRIs) and other new antidepressants, such as buproprion and venlafaxine, are generally considered to be the first-line choices for the depressed phase of bipolar disease.	topic_bd
76648	4	355671	7	NULL	NULL	0	NULL	buproprion	Chemical		first-line choice					bipolar disease	MedicalFinding	for the depressed phase of			NULL		0	NULL	NULL	NULL	NULL	NULL	Selective serotonin reuptake inhibitors (SSRIs) and other new antidepressants, such as buproprion and venlafaxine, are generally considered to be the first-line choices for the depressed phase of bipolar disease.	topic_bd
76649	5	355671	7	NULL	NULL	0	NULL	venlafaxine	Chemical		first-line choice					bipolar disease	MedicalFinding	for the depressed phase of			NULL		0	NULL	NULL	NULL	NULL	NULL	Selective serotonin reuptake inhibitors (SSRIs) and other new antidepressants, such as buproprion and venlafaxine, are generally considered to be the first-line choices for the depressed phase of bipolar disease.	topic_bd
76650	6	355671	7	NULL	NULL	0	NULL	SSRI	Chemical		is					Selective serotonin reuptake inhibitors	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Selective serotonin reuptake inhibitors (SSRIs) and other new antidepressants, such as buproprion and venlafaxine, are generally considered to be the first-line choices for the depressed phase of bipolar disease.	topic_bd
76651	1	355672	7	NULL	NULL	0	NULL	SSRI	Chemical		induce					mania	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mania or hypomania is a possible side effect. Users with some type of bipolar disorder are at a much higher risk, however SSRI-induced mania in patients previously diagnosed with unipolar depression can trigger a bipolar diagnosis.	topic_bd
76652	2	355672	7	NULL	NULL	0	NULL	statement 1	Process		occur in					unipolar depression	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mania or hypomania is a possible side effect. Users with some type of bipolar disorder are at a much higher risk, however SSRI-induced mania in patients previously diagnosed with unipolar depression can trigger a bipolar diagnosis.	topic_bd
76653	3	355672	7	NULL	NULL	0	NULL	statement 1	Process		trigger		could			bipolar depression	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mania or hypomania is a possible side effect. Users with some type of bipolar disorder are at a much higher risk, however SSRI-induced mania in patients previously diagnosed with unipolar depression can trigger a bipolar diagnosis.	topic_bd
76654	1	355673	7	NULL	NULL	0	NULL	lithium	Chemical		act through		potentially			GSK3	GP	inhibition of			NULL		0	NULL	NULL	NULL	NULL	NULL	Since lithium has been shown to potentially act through glycogen synthase kinase-3 (GSK3) inhibition, we evaluated the efficacy of selective GSK3 inhibitors in this model.	topic_bd
76655	2	355673	7	NULL	NULL	NULL	NULL	GSK3	GP		is					glycogen synthase kinase-3	GP				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Since lithium has been shown to potentially act through glycogen synthase kinase-3 (GSK3) inhibition, we evaluated the efficacy of selective GSK3 inhibitors in this model.	topic_bd
76656	1	355674	7	NULL	NULL	0	NULL	DISC1gene	GP		associated with					schizophrenia	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	The Disrupted in Schizophrenia 1 (DISC1) gene has been associated with the risk of schizophrenia, schizoaffective disorder, bipolar disorder, major depression, autism, and Asperger syndrome in different populations.	topic_bd
76657	2	355674	7	NULL	NULL	0	NULL	DISC1gene	GP		associated with					schizoaffective disorder	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	The Disrupted in Schizophrenia 1 (DISC1) gene has been associated with the risk of schizophrenia, schizoaffective disorder, bipolar disorder, major depression, autism, and Asperger syndrome in different populations.	topic_bd
76658	3	355674	7	NULL	NULL	0	NULL	DISC1gene	GP		associated with					bipolar disorder	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	The Disrupted in Schizophrenia 1 (DISC1) gene has been associated with the risk of schizophrenia, schizoaffective disorder, bipolar disorder, major depression, autism, and Asperger syndrome in different populations.	topic_bd
76659	4	355674	7	NULL	NULL	0	NULL	DISC1gene	GP		associated with					major depression	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	The Disrupted in Schizophrenia 1 (DISC1) gene has been associated with the risk of schizophrenia, schizoaffective disorder, bipolar disorder, major depression, autism, and Asperger syndrome in different populations.	topic_bd
76660	5	355674	7	NULL	NULL	0	NULL	DISC1gene	GP		associated with					autism	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	The Disrupted in Schizophrenia 1 (DISC1) gene has been associated with the risk of schizophrenia, schizoaffective disorder, bipolar disorder, major depression, autism, and Asperger syndrome in different populations.	topic_bd
76661	6	355674	7	NULL	NULL	0	NULL	DISC1gene	GP		associated with					Asperger syndrome	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	The Disrupted in Schizophrenia 1 (DISC1) gene has been associated with the risk of schizophrenia, schizoaffective disorder, bipolar disorder, major depression, autism, and Asperger syndrome in different populations.	topic_bd
76662	7	355674	7	NULL	NULL	0	NULL	DISC1gene	GP		is					Disrupted in Schizophrenia 1	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The Disrupted in Schizophrenia 1 (DISC1) gene has been associated with the risk of schizophrenia, schizoaffective disorder, bipolar disorder, major depression, autism, and Asperger syndrome in different populations.	topic_bd
76663	1	355675	7	NULL	NULL	0	NULL	MDR1 gene	GP	Polymorphism in the	occur in					colon cancer 	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphism in the P-glycoprotein drug transporter MDR1 gene in colon cancer patients. 	topic_ccc
76664	2	355675	7	NULL	NULL	0	NULL	MDR1 gene	GP		is a type of					P-glycoprotein drug transporter	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphism in the P-glycoprotein drug transporter MDR1 gene in colon cancer patients. 	topic_ccc
76665	1	355677	7	NULL	NULL	NULL	NULL	MDR1 gene	GP	polymorphism of	associated with					colon cancer	MedicalFinding	occurence of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	 In the present study, an association of MDR1 gene polymorphism and the occurrence of colon cancer were evaluated.	topic_ccc
76666	1	355678	7	NULL	NULL	0	NULL	SN-38 	Chemical		active metabolite of					irinotecan	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	SN-38 is an active metabolite of the topoisomerase I inhibitor irinotecan. The mechanism behind its antitumor effect in colorectal cancer is not fully understood. 	topic_ccc
76667	2	355678	7	NULL	NULL	0	NULL	irinotecan	Chemical		is a type of					topoisomerase I inhibitor	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	SN-38 is an active metabolite of the topoisomerase I inhibitor irinotecan. The mechanism behind its antitumor effect in colorectal cancer is not fully understood. 	topic_ccc
76668	3	355678	7	NULL	NULL	0	NULL	SN-38	Chemical		possess					colorectal cancer	MedicalFinding	antitumor effect in			NULL		0	NULL	NULL	NULL	NULL	NULL	SN-38 is an active metabolite of the topoisomerase I inhibitor irinotecan. The mechanism behind its antitumor effect in colorectal cancer is not fully understood. 	topic_ccc
75960	1	355679	5	NULL	NULL	0	NULL	macrocephaly	MedicalFinding		is present in					autistic children	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Research indicates the presence of macrocephaly or abnormally large head circumferences in children with autism and spectrum-related disorders, compared with their typically developing peers	topic_aut
75961	2	355679	5	NULL	NULL	0	NULL	macrocephaly	MedicalFinding		is present in					spectrum-related disorder children	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Research indicates the presence of macrocephaly or abnormally large head circumferences in children with autism and spectrum-related disorders, compared with their typically developing peers	topic_aut
75962	3	355679	5	NULL	NULL	0	NULL	macrocephaly	MedicalFinding		is a synonym of					abnormally large head circumference	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Research indicates the presence of macrocephaly or abnormally large head circumferences in children with autism and spectrum-related disorders, compared with their typically developing peers	topic_aut
75998	1	355680	5	NULL	NULL	0	NULL	synaptic genes	GP	alternation of	plays a role in		important			ASD	MedicalFinding	pathogenesis of			NULL		0	NULL	NULL	NULL	NULL	NULL	Recent genetic studies demonstrate that alterations in synaptic genes including those encoding cell adhesion molecules and their interaction partners play important roles in the pathogenesis of ASD	topic_aut
75999	2	355680	5	NULL	NULL	0	NULL	synaptic genes	GP		include					cell adhesion molecules	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Recent genetic studies demonstrate that alterations in synaptic genes including those encoding cell adhesion molecules and their interaction partners play important roles in the pathogenesis of ASD	topic_aut
76000	1	355681	5	NULL	NULL	0	NULL	autistic individuals	GroupOfPeople		use					emotion processing	Process	multiple routes of 			NULL		0	NULL	NULL	NULL	NULL	NULL	I elaborate on this model by discussing recent research on emotional recognition in individuals with autism, who can use multiple routes of emotion processing, and consequently can show atypical and typical patterns of embodied simulation and mimicry.	topic_aut
76001	2	355681	5	NULL	NULL	0	NULL	statement 1	Process		leads to		consequetly			embodied simulation	Process	atypical patterns of			NULL		0	NULL	NULL	NULL	NULL	NULL	I elaborate on this model by discussing recent research on emotional recognition in individuals with autism, who can use multiple routes of emotion processing, and consequently can show atypical and typical patterns of embodied simulation and mimicry.	topic_aut
76002	3	355681	5	NULL	NULL	0	NULL	statement 1	Process		leads to		consequetly			mimicry	Process	atypical patterns of			NULL		0	NULL	NULL	NULL	NULL	NULL	I elaborate on this model by discussing recent research on emotional recognition in individuals with autism, who can use multiple routes of emotion processing, and consequently can show atypical and typical patterns of embodied simulation and mimicry.	topic_aut
76003	4	355681	5	NULL	NULL	0	NULL	statement 1	Process		leads to		consequetly			embodied simulation	Process	typical patterns of			NULL		0	NULL	NULL	NULL	NULL	NULL	I elaborate on this model by discussing recent research on emotional recognition in individuals with autism, who can use multiple routes of emotion processing, and consequently can show atypical and typical patterns of embodied simulation and mimicry.	topic_aut
76004	5	355681	5	NULL	NULL	0	NULL	statement 1	Process		leads to		consequetly			mimicry	Process	typical patterns of			NULL		0	NULL	NULL	NULL	NULL	NULL	I elaborate on this model by discussing recent research on emotional recognition in individuals with autism, who can use multiple routes of emotion processing, and consequently can show atypical and typical patterns of embodied simulation and mimicry.	topic_aut
76005	1	355682	5	NULL	NULL	0	NULL	pregnancy	MedicalFinding	complications of 	implicate					fetal hypoxia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Autism spectrum disorders (ASD) are associated with complications of pregnancy that implicate fetal hypoxia (FH)	topic_aut
76006	2	355682	5	NULL	NULL	0	NULL	FH	MedicalFinding		is					fetal hypoxia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Autism spectrum disorders (ASD) are associated with complications of pregnancy that implicate fetal hypoxia (FH)	topic_aut
76007	3	355682	5	NULL	NULL	0	NULL	ASD	MedicalFinding		is					autism spectrum disorders	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Autism spectrum disorders (ASD) are associated with complications of pregnancy that implicate fetal hypoxia (FH)	topic_aut
76008	4	355682	5	NULL	NULL	0	NULL	ASD	MedicalFinding		is associated with					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Autism spectrum disorders (ASD) are associated with complications of pregnancy that implicate fetal hypoxia (FH)	topic_aut
76009	1	355684	5	NULL	NULL	0	NULL	thimerosal	Chemical		is a type of					mercurial	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	These findings document neurotoxic effects of thimerosal, at doses equivalent to those used in infant vaccines or higher, in developing rat brain, suggesting likely involvement of this mercurial in neurodevelopmental disorders	topic_aut
76010	2	355684	5	NULL	NULL	0	NULL	thimerosal	Chemical		is involved in					neurodevelopmental disorders	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	These findings document neurotoxic effects of thimerosal, at doses equivalent to those used in infant vaccines or higher, in developing rat brain, suggesting likely involvement of this mercurial in neurodevelopmental disorders	topic_aut
76011	1	355686	5	NULL	NULL	0	NULL	porphyrin	Chemical	disordered metabolism of	is a characteristic of		salient			autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	These findings identify disordered porphyrin metabolism as a salient characteristic of autism.	topic_aut
76012	1	355687	5	NULL	NULL	0	NULL	familial platelet disorder 	MedicalFinding		confers susceptibility to					acute myelogenous leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Gilliland and his colleagues have identified genetic mutations that cause a familial platelet disorder that confers susceptibility to acute myelogenous leukemia (AML).	topic_ll
76013	2	355687	5	NULL	NULL	0	NULL	acute myelogenous leukemia	MedicalFinding		is					AML	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Gilliland and his colleagues have identified genetic mutations that cause a familial platelet disorder that confers susceptibility to acute myelogenous leukemia (AML).	topic_ll
76014	1	355688	5	NULL	NULL	0	NULL	CBFA2 protein	GP		activates					blood cell	Cell	development of			NULL		0	NULL	NULL	NULL	NULL	NULL	Looking more closely at that region of chromosome 21, the researchers found a mutation in the gene, CBFA2, which produces a protein that activates blood cell development.	topic_ll
76015	2	355688	5	NULL	NULL	0	NULL	CBFA2 gene	GP		is present in					chromosome 21	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	Looking more closely at that region of chromosome 21, the researchers found a mutation in the gene, CBFA2, which produces a protein that activates blood cell development.	topic_ll
76016	1	355689	5	NULL	NULL	0	NULL	chromosomes	Chromosome		swap		inappropriately			genetic material	NucleicAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	Leukemias and lymphomas can arise when chromosomes inappropriately swap genetic material.	topic_ll
76017	2	355689	5	NULL	NULL	0	NULL	statement 1	Process		leads to					leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Leukemias and lymphomas can arise when chromosomes inappropriately swap genetic material.	topic_ll
76018	3	355689	5	NULL	NULL	0	NULL	statement 1	Process		leads to					lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Leukemias and lymphomas can arise when chromosomes inappropriately swap genetic material.	topic_ll
76019	1	355691	5	NULL	NULL	0	NULL	gene	GP	complex translocation of	leads to					genome	Chromosome	amplification of;;large regions of 			NULL		0	NULL	NULL	NULL	NULL	NULL	In some cases, more complex gene translocations (as opposed to swapping one gene for another) lead to amplification of large regions of the genome. Alt and his colleagues coined the term complicon—derived from complex translocation—to describe this phenomenon. 	topic_ll
76020	2	355691	5	NULL	NULL	0	NULL	statement 1	Process		is termed					complicon	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	In some cases, more complex gene translocations (as opposed to swapping one gene for another) lead to amplification of large regions of the genome. Alt and his colleagues coined the term complicon—derived from complex translocation—to describe this phenomenon. 	topic_ll
76021	1	355693	5	NULL	NULL	0	NULL	lymphoma	MedicalFinding		is a type of					blood cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In the 1970s, clinicians noted that the blood cancer lymphoma was also very common in boys with XLP. “	topic_ll
76022	2	355693	5	NULL	NULL	0	NULL	lymphoma	MedicalFinding		is common in					XLP boys	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	In the 1970s, clinicians noted that the blood cancer lymphoma was also very common in boys with XLP. “	topic_ll
76023	1	355694	5	NULL	NULL	0	NULL	XLP	MedicalFinding		is					X-linked lymphoproliferative disease	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The findings, published on August 2, 2009 in Nature Immunology, may also lead to better understanding of a rare genetic disorder called X-linked lymphoproliferative disease (XLP), which causes the immune system to go into overdrive. 	topic_ll
76024	2	355694	5	NULL	NULL	0	NULL	XLP	MedicalFinding		is a type of					rare genetic disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The findings, published on August 2, 2009 in Nature Immunology, may also lead to better understanding of a rare genetic disorder called X-linked lymphoproliferative disease (XLP), which causes the immune system to go into overdrive. 	topic_ll
76025	3	355694	5	NULL	NULL	0	NULL	XLP	MedicalFinding		overdrives					immune system	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	The findings, published on August 2, 2009 in Nature Immunology, may also lead to better understanding of a rare genetic disorder called X-linked lymphoproliferative disease (XLP), which causes the immune system to go into overdrive. 	topic_ll
76026	1	355695	5	NULL	NULL	0	NULL	natural killer cells	Cell		lacks					SAP-related molecules	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Further experiments in live mice confirmed that the natural killer cells lacking the SAP-related molecules were unable to kill lymphoma cells. 	topic_ll
76027	2	355695	5	NULL	NULL	0	NULL	statement 1	Process		unable to kill					lymphoma cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Further experiments in live mice confirmed that the natural killer cells lacking the SAP-related molecules were unable to kill lymphoma cells. 	topic_ll
76028	1	355696	5	NULL	NULL	0	NULL	SAP	GP		is					SLAM-Associated Protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	molecules interact with SAP (which stands for SLAM-Associated Protein), but no one understood what role SAP played in commanding the immune system’s assassins to attack. 	topic_ll
76029	2	355696	5	NULL	NULL	0	NULL	immune system assassins	GP		is commanded to					attack	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	molecules interact with SAP (which stands for SLAM-Associated Protein), but no one understood what role SAP played in commanding the immune system’s assassins to attack. 	topic_ll
76030	3	355696	5	NULL	NULL	0	NULL	SAP	GP		plays a role in		possibly			statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	molecules interact with SAP (which stands for SLAM-Associated Protein), but no one understood what role SAP played in commanding the immune system’s assassins to attack. 	topic_ll
76031	1	355697	5	NULL	NULL	0	NULL	mycosis fungoides	MedicalFinding		is also known as					Alibert-Bazin syndrome	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mycosis fungoides (also known as Alibert-Bazin syndrome or granuloma fungoides), is the most common form of cutaneous T-cell lymphoma.	topic_ll
76032	2	355697	5	NULL	NULL	0	NULL	mycosis fungoides	MedicalFinding		is also known as					granuloma fungoides	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mycosis fungoides (also known as Alibert-Bazin syndrome or granuloma fungoides), is the most common form of cutaneous T-cell lymphoma.	topic_ll
76033	3	355697	5	NULL	NULL	0	NULL	mycosis fungoides	MedicalFinding		is a form of		most common			cutaneous T-cell lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mycosis fungoides (also known as Alibert-Bazin syndrome or granuloma fungoides), is the most common form of cutaneous T-cell lymphoma.	topic_ll
76034	1	355699	5	NULL	NULL	0	NULL	lymphocyte	Cell		is a type of					white blood cell	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Mycosis fungoides and the Sézary syndrome are diseases in which lymphocytes (a type of white blood cell) become malignant (cancerous) and affect the skin.	topic_ll
76035	2	355699	5	NULL	NULL	0	NULL	 lymphocyte	Cell		become					malignant	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mycosis fungoides and the Sézary syndrome are diseases in which lymphocytes (a type of white blood cell) become malignant (cancerous) and affect the skin.	topic_ll
76036	3	355699	5	NULL	NULL	0	NULL	statement 2	Process		affects					skin	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Mycosis fungoides and the Sézary syndrome are diseases in which lymphocytes (a type of white blood cell) become malignant (cancerous) and affect the skin.	topic_ll
76037	4	355699	5	NULL	NULL	0	NULL	malignant	MedicalFinding		is also known as					cancerous	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mycosis fungoides and the Sézary syndrome are diseases in which lymphocytes (a type of white blood cell) become malignant (cancerous) and affect the skin.	topic_ll
76038	5	355699	5	NULL	NULL	0	NULL	mycosis fungoides	MedicalFinding		leads to					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Mycosis fungoides and the Sézary syndrome are diseases in which lymphocytes (a type of white blood cell) become malignant (cancerous) and affect the skin.	topic_ll
76039	6	355699	5	NULL	NULL	0	NULL	Sézary syndrome	MedicalFinding		leads to					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Mycosis fungoides and the Sézary syndrome are diseases in which lymphocytes (a type of white blood cell) become malignant (cancerous) and affect the skin.	topic_ll
76040	1	355700	5	NULL	NULL	0	NULL	Pagetoid reticulosis of Woringer-Kolopp	MedicalFinding		is a form of		rare			cutaneous T-cell lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Pagetoid reticulosis of Woringer-Kolopp is a rare form of cutaneous T-cell lymphoma that primarily affects middle-aged males.	topic_ll
76041	2	355700	5	NULL	NULL	0	NULL	cutaneous T-cell lymphoma	MedicalFinding		affects		primarily			middle-aged males	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Pagetoid reticulosis of Woringer-Kolopp is a rare form of cutaneous T-cell lymphoma that primarily affects middle-aged males.	topic_ll
76053	1	355701	5	NULL	NULL	0	NULL	Pagetoid reticulosis of Woringer-Kolopp	MedicalFinding		is a form of		rare			cutaneous T-cell lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Pagetoid reticulosis of Woringer-Kolopp is a rare form of cutaneous T-cell lymphoma that primarily affects middle-aged males. It is characterized by the presence of one or several scaly patches and plaques with an acral distribution.	topic_ll
76054	2	355701	5	NULL	NULL	0	NULL	statement 1	MedicalFinding		affects		primarily			middle-aged males	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Pagetoid reticulosis of Woringer-Kolopp is a rare form of cutaneous T-cell lymphoma that primarily affects middle-aged males. It is characterized by the presence of one or several scaly patches and plaques with an acral distribution.	topic_ll
76055	3	355701	5	NULL	NULL	0	NULL	statement 1	MedicalFinding		is characterized by					scaly patches	MedicalFinding	presence of			NULL		0	NULL	NULL	NULL	NULL	NULL	Pagetoid reticulosis of Woringer-Kolopp is a rare form of cutaneous T-cell lymphoma that primarily affects middle-aged males. It is characterized by the presence of one or several scaly patches and plaques with an acral distribution.	topic_ll
76056	4	355701	5	NULL	NULL	0	NULL	statement 1	MedicalFinding		is characterized by					plaques	MedicalFinding	presence of			NULL		0	NULL	NULL	NULL	NULL	NULL	Pagetoid reticulosis of Woringer-Kolopp is a rare form of cutaneous T-cell lymphoma that primarily affects middle-aged males. It is characterized by the presence of one or several scaly patches and plaques with an acral distribution.	topic_ll
76057	5	355701	5	NULL	NULL	0	NULL	scaly patches	MedicalFinding		is distributed					acrally	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Pagetoid reticulosis of Woringer-Kolopp is a rare form of cutaneous T-cell lymphoma that primarily affects middle-aged males. It is characterized by the presence of one or several scaly patches and plaques with an acral distribution.	topic_ll
76058	6	355701	5	NULL	NULL	0	NULL	plaques	MedicalFinding		is distributed					acrally	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Pagetoid reticulosis of Woringer-Kolopp is a rare form of cutaneous T-cell lymphoma that primarily affects middle-aged males. It is characterized by the presence of one or several scaly patches and plaques with an acral distribution.	topic_ll
76059	1	355702	5	NULL	NULL	0	NULL	pagetoid reticulosis	MedicalFinding	localized	is a type of					polycyclic erythematous scaly lesions	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Localized pagetoid reticulosis is an uncommon disease described by Woringer and Kolopp in 1939 as "polycyclic erythematous scaly lesions with 6-year evolution on the forearm of 13-year-old boy" [1]. 	topic_ll
76060	2	355702	5	NULL	NULL	0	NULL	pagetoid reticulosis	MedicalFinding	localized	identified by					Woringer and Kolopp	Person				NULL		0	NULL	NULL	NULL	NULL	NULL	Localized pagetoid reticulosis is an uncommon disease described by Woringer and Kolopp in 1939 as "polycyclic erythematous scaly lesions with 6-year evolution on the forearm of 13-year-old boy" [1]. 	topic_ll
76061	1	355703	5	NULL	NULL	0	NULL	Pagetoid reticulosis	MedicalFinding		features					lesions	MedicalFinding	acral distribution of			NULL		0	NULL	NULL	NULL	NULL	NULL	Pagetoid reticulosis features acral distribution of lesions, pronounced hyperkeratosis and acanthosis, prominent epidermotropism, and expression of a cutaneous lymphocyte antigen 	topic_ll
76062	2	355703	5	NULL	NULL	0	NULL	Pagetoid reticulosis	MedicalFinding		features					hyperkeratosis	MedicalFinding	pronounced			NULL		0	NULL	NULL	NULL	NULL	NULL	Pagetoid reticulosis features acral distribution of lesions, pronounced hyperkeratosis and acanthosis, prominent epidermotropism, and expression of a cutaneous lymphocyte antigen 	topic_ll
76063	3	355703	5	NULL	NULL	0	NULL	Pagetoid reticulosis	MedicalFinding		features					acanthosis	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Pagetoid reticulosis features acral distribution of lesions, pronounced hyperkeratosis and acanthosis, prominent epidermotropism, and expression of a cutaneous lymphocyte antigen 	topic_ll
76064	4	355703	5	NULL	NULL	0	NULL	Pagetoid reticulosis	MedicalFinding		features					epidermotropism	MedicalFinding	prominent			NULL		0	NULL	NULL	NULL	NULL	NULL	Pagetoid reticulosis features acral distribution of lesions, pronounced hyperkeratosis and acanthosis, prominent epidermotropism, and expression of a cutaneous lymphocyte antigen 	topic_ll
76065	5	355703	5	NULL	NULL	0	NULL	Pagetoid reticulosis	MedicalFinding		features					cutaneous lymphocyte antigen	GP	 expression of			NULL		0	NULL	NULL	NULL	NULL	NULL	Pagetoid reticulosis features acral distribution of lesions, pronounced hyperkeratosis and acanthosis, prominent epidermotropism, and expression of a cutaneous lymphocyte antigen 	topic_ll
76066	1	355704	5	NULL	NULL	0	NULL	GSS	MedicalFinding		is					granulomatous slack skin	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Granulomatous slack skin (GSS) is a rare cutaneous disorder characterized clinically by the evolution of circumscribed erythematous lax skin masses, especially in the body folds, and histologically by a granulomatous T-cell infiltrate and loss of elastic fibers.	topic_ll
76067	2	355704	5	NULL	NULL	0	NULL	granulomatous slack skin\t\t	MedicalFinding		is a type of					rare cutaneous disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Granulomatous slack skin (GSS) is a rare cutaneous disorder characterized clinically by the evolution of circumscribed erythematous lax skin masses, especially in the body folds, and histologically by a granulomatous T-cell infiltrate and loss of elastic fibers.	topic_ll
76068	3	355704	5	NULL	NULL	NULL	NULL	GSS	MedicalFinding		is characterized by		clinically			erythematous lax skin masses	MedicalFinding	evolution of;;circumscribed			NULL	body folds	NULL	NULL	NULL	NULL	NULL	NULL	Granulomatous slack skin (GSS) is a rare cutaneous disorder characterized clinically by the evolution of circumscribed erythematous lax skin masses, especially in the body folds, and histologically by a granulomatous T-cell infiltrate and loss of elastic fibers.	topic_ll
76069	4	355704	5	NULL	NULL	0	NULL	GSS	MedicalFinding		is characterized by		histologically			granulomatous T-cell infiltrate	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Granulomatous slack skin (GSS) is a rare cutaneous disorder characterized clinically by the evolution of circumscribed erythematous lax skin masses, especially in the body folds, and histologically by a granulomatous T-cell infiltrate and loss of elastic fibers.	topic_ll
76070	5	355704	5	NULL	NULL	NULL	NULL	GSS	MedicalFinding		is characterized by					elastic fibers	CellComponent	loss of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Granulomatous slack skin (GSS) is a rare cutaneous disorder characterized clinically by the evolution of circumscribed erythematous lax skin masses, especially in the body folds, and histologically by a granulomatous T-cell infiltrate and loss of elastic fibers.	topic_ll
76071	1	355705	5	NULL	NULL	0	NULL	GSS	MedicalFinding		is associated with					lymphoproliferative malignancies	MedicalFinding	preceding			NULL		0	NULL	NULL	NULL	NULL	NULL	GSS is often associated with preceding or subsequent lymphoproliferative malignancies, especially mycosis fungoides (MF) and Hodgkin's disease (HD). 	topic_ll
76072	2	355705	5	NULL	NULL	0	NULL	GSS	MedicalFinding		is associated with					lymphoproliferative malignancies	MedicalFinding	subsequent			NULL		0	NULL	NULL	NULL	NULL	NULL	GSS is often associated with preceding or subsequent lymphoproliferative malignancies, especially mycosis fungoides (MF) and Hodgkin's disease (HD). 	topic_ll
76073	3	355705	5	NULL	NULL	0	NULL	MF	MedicalFinding		is					mycosis fungoides	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	GSS is often associated with preceding or subsequent lymphoproliferative malignancies, especially mycosis fungoides (MF) and Hodgkin's disease (HD). 	topic_ll
76074	4	355705	5	NULL	NULL	0	NULL	HD	MedicalFinding		is					Hodgkin's disease	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	GSS is often associated with preceding or subsequent lymphoproliferative malignancies, especially mycosis fungoides (MF) and Hodgkin's disease (HD). 	topic_ll
76075	5	355705	5	NULL	NULL	0	NULL	MF	MedicalFinding		is a type of					lymphoproliferative malignancies	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	GSS is often associated with preceding or subsequent lymphoproliferative malignancies, especially mycosis fungoides (MF) and Hodgkin's disease (HD). 	topic_ll
76076	6	355705	5	NULL	NULL	0	NULL	HD	MedicalFinding		is a type of					lymphoproliferative malignancies	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	GSS is often associated with preceding or subsequent lymphoproliferative malignancies, especially mycosis fungoides (MF) and Hodgkin's disease (HD). 	topic_ll
76089	7	355705	5	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	GSS is often associated with preceding or subsequent lymphoproliferative malignancies, especially mycosis fungoides (MF) and Hodgkin's disease (HD). 	topic_ll
76077	1	355706	5	NULL	NULL	0	NULL	elastic fibers	CellComponent	disappearance of	results in					lax skin	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Apparently, the disease is associated with a peculiar immune response, characterized by granuloma formation and disappearance of elastic fibers resulting in the lax skin. 	topic_ll
76078	1	355708	5	NULL	NULL	0	NULL	Bexarotene capsules	Chemical		slow					CTCL tumors	MedicalFinding	growth of;;large			NULL		0	NULL	NULL	NULL	NULL	NULL	Bexarotene capsules Bexarotene in capsule form can slow or stall the growth of large CTCL tumors. The patient ingests the pill with food daily.	topic_ll
76079	2	355708	5	NULL	NULL	0	NULL	Bexarotene capsules	Chemical		stall					CTCL tumors	MedicalFinding	growth of;;large			NULL		0	NULL	NULL	NULL	NULL	NULL	Bexarotene capsules Bexarotene in capsule form can slow or stall the growth of large CTCL tumors. The patient ingests the pill with food daily.	topic_ll
76080	3	355708	5	NULL	NULL	0	NULL	Bexarotene capsules	Chemical		is ingested with					food	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Bexarotene capsules Bexarotene in capsule form can slow or stall the growth of large CTCL tumors. The patient ingests the pill with food daily.	topic_ll
76081	1	355709	5	NULL	NULL	0	NULL	PUVA treatment	MedicalProcedure		is also known as					photochemotherapy	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Also known as photochemotherapy, PUVA treatment is successful in treating CTCL where large areas of the skin are affected.	topic_ll
76082	2	355709	5	NULL	NULL	0	NULL	PUVA treatment	MedicalProcedure		is used to treat		successfully			CTCL	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Also known as photochemotherapy, PUVA treatment is successful in treating CTCL where large areas of the skin are affected.	topic_ll
76083	3	355709	5	NULL	NULL	0	NULL	CTCL	MedicalFinding		affects					skin	OrganismPart	large areas of			NULL		0	NULL	NULL	NULL	NULL	NULL	Also known as photochemotherapy, PUVA treatment is successful in treating CTCL where large areas of the skin are affected.	topic_ll
76084	1	355710	5	NULL	NULL	0	NULL	psoralen	Chemical		is a type of					drug	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The patient takes a drug called psoralen (P), which makes the skin sensitive to Ultraviolet A light rays. The UVA then attacks cancerous cells.	topic_ll
76085	2	355710	5	NULL	NULL	0	NULL	skin	OrganismPart		is made sensitive to					Ultraviolet A light rays	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	NULL	NULL	The patient takes a drug called psoralen (P), which makes the skin sensitive to Ultraviolet A light rays. The UVA then attacks cancerous cells.	topic_ll
76086	3	355710	5	NULL	NULL	0	NULL	psoralen	Chemical		plays a role in					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The patient takes a drug called psoralen (P), which makes the skin sensitive to Ultraviolet A light rays. The UVA then attacks cancerous cells.	topic_ll
76087	4	355710	5	NULL	NULL	0	NULL	UVA	PhysicalPhenomenon		attacks					cancerous cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	The patient takes a drug called psoralen (P), which makes the skin sensitive to Ultraviolet A light rays. The UVA then attacks cancerous cells.	topic_ll
76088	5	355710	5	NULL	NULL	0	NULL	statement 2	Process		is followed by					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The patient takes a drug called psoralen (P), which makes the skin sensitive to Ultraviolet A light rays. The UVA then attacks cancerous cells.	topic_ll
76090	1	355712	5	NULL	NULL	0	NULL	blood	OrganismPart		is removed from 					patient	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Photopheresis Pheresis treatments involve removing blood from a patient, cycling it through a machine to clean or treat it, and then returning it to the patient. For Sézary Syndrome patients, the blood is exposed to UV light before it is returned to the body. This helps remove affected T-cells from the blood.	topic_ll
76091	2	355712	5	NULL	NULL	0	NULL	blood	OrganismPart		is cycled through					machine	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Photopheresis Pheresis treatments involve removing blood from a patient, cycling it through a machine to clean or treat it, and then returning it to the patient. For Sézary Syndrome patients, the blood is exposed to UV light before it is returned to the body. This helps remove affected T-cells from the blood.	topic_ll
76092	3	355712	5	NULL	NULL	0	NULL	statement 1	Process		is followed by					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Photopheresis Pheresis treatments involve removing blood from a patient, cycling it through a machine to clean or treat it, and then returning it to the patient. For Sézary Syndrome patients, the blood is exposed to UV light before it is returned to the body. This helps remove affected T-cells from the blood.	topic_ll
76093	13	355712	5	NULL	NULL	NULL	NULL	Pheresis treatment	MedicalProcedure		involves					statement 1	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Photopheresis Pheresis treatments involve removing blood from a patient, cycling it through a machine to clean or treat it, and then returning it to the patient. For Sézary Syndrome patients, the blood is exposed to UV light before it is returned to the body. This helps remove affected T-cells from the blood.	topic_ll
76094	14	355712	5	NULL	NULL	NULL	NULL	Pheresis treatment	MedicalProcedure		involves					statement 2	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Photopheresis Pheresis treatments involve removing blood from a patient, cycling it through a machine to clean or treat it, and then returning it to the patient. For Sézary Syndrome patients, the blood is exposed to UV light before it is returned to the body. This helps remove affected T-cells from the blood.	topic_ll
76095	4	355712	5	NULL	NULL	0	NULL	statement 2	Process		cleans					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Photopheresis Pheresis treatments involve removing blood from a patient, cycling it through a machine to clean or treat it, and then returning it to the patient. For Sézary Syndrome patients, the blood is exposed to UV light before it is returned to the body. This helps remove affected T-cells from the blood.	topic_ll
76096	5	355712	5	NULL	NULL	NULL	NULL	statement 2	Process		treats					statement 1	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Photopheresis Pheresis treatments involve removing blood from a patient, cycling it through a machine to clean or treat it, and then returning it to the patient. For Sézary Syndrome patients, the blood is exposed to UV light before it is returned to the body. This helps remove affected T-cells from the blood.	topic_ll
76097	6	355712	5	NULL	NULL	0	NULL	statement 4	Process		is an alternative to					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Photopheresis Pheresis treatments involve removing blood from a patient, cycling it through a machine to clean or treat it, and then returning it to the patient. For Sézary Syndrome patients, the blood is exposed to UV light before it is returned to the body. This helps remove affected T-cells from the blood.	topic_ll
76098	7	355712	5	NULL	NULL	0	NULL	blood	OrganismPart	cleaned	returned to					patient	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Photopheresis Pheresis treatments involve removing blood from a patient, cycling it through a machine to clean or treat it, and then returning it to the patient. For Sézary Syndrome patients, the blood is exposed to UV light before it is returned to the body. This helps remove affected T-cells from the blood.	topic_ll
76099	8	355712	5	NULL	NULL	0	NULL	blood	OrganismPart	treated	returned to					patient	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Photopheresis Pheresis treatments involve removing blood from a patient, cycling it through a machine to clean or treat it, and then returning it to the patient. For Sézary Syndrome patients, the blood is exposed to UV light before it is returned to the body. This helps remove affected T-cells from the blood.	topic_ll
76100	9	355712	5	NULL	NULL	0	NULL	statement 2	Process		is followed by					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Photopheresis Pheresis treatments involve removing blood from a patient, cycling it through a machine to clean or treat it, and then returning it to the patient. For Sézary Syndrome patients, the blood is exposed to UV light before it is returned to the body. This helps remove affected T-cells from the blood.	topic_ll
76101	10	355712	5	NULL	NULL	0	NULL	statement 2	Process		is followed by					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Photopheresis Pheresis treatments involve removing blood from a patient, cycling it through a machine to clean or treat it, and then returning it to the patient. For Sézary Syndrome patients, the blood is exposed to UV light before it is returned to the body. This helps remove affected T-cells from the blood.	topic_ll
76102	11	355712	5	NULL	NULL	0	NULL	statement 9	Process		is followed by					statement 7	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Photopheresis Pheresis treatments involve removing blood from a patient, cycling it through a machine to clean or treat it, and then returning it to the patient. For Sézary Syndrome patients, the blood is exposed to UV light before it is returned to the body. This helps remove affected T-cells from the blood.	topic_ll
76103	12	355712	5	NULL	NULL	0	NULL	statement 10	Process		is followed by					statement 8	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Photopheresis Pheresis treatments involve removing blood from a patient, cycling it through a machine to clean or treat it, and then returning it to the patient. For Sézary Syndrome patients, the blood is exposed to UV light before it is returned to the body. This helps remove affected T-cells from the blood.	topic_ll
76104	15	355712	5	NULL	NULL	0	NULL	Pheresis treatment	MedicalProcedure		involves					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Photopheresis Pheresis treatments involve removing blood from a patient, cycling it through a machine to clean or treat it, and then returning it to the patient. For Sézary Syndrome patients, the blood is exposed to UV light before it is returned to the body. This helps remove affected T-cells from the blood.	topic_ll
76105	16	355712	5	NULL	NULL	0	NULL	Pheresis treatment	MedicalProcedure		involves					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Photopheresis Pheresis treatments involve removing blood from a patient, cycling it through a machine to clean or treat it, and then returning it to the patient. For Sézary Syndrome patients, the blood is exposed to UV light before it is returned to the body. This helps remove affected T-cells from the blood.	topic_ll
76106	17	355712	5	NULL	NULL	0	NULL	Pheresis treatment	MedicalProcedure		involves					statement 7	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Photopheresis Pheresis treatments involve removing blood from a patient, cycling it through a machine to clean or treat it, and then returning it to the patient. For Sézary Syndrome patients, the blood is exposed to UV light before it is returned to the body. This helps remove affected T-cells from the blood.	topic_ll
76107	18	355712	5	NULL	NULL	0	NULL	Pheresis treatment	MedicalProcedure		involves					statement 8	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Photopheresis Pheresis treatments involve removing blood from a patient, cycling it through a machine to clean or treat it, and then returning it to the patient. For Sézary Syndrome patients, the blood is exposed to UV light before it is returned to the body. This helps remove affected T-cells from the blood.	topic_ll
76108	19	355712	5	NULL	NULL	NULL	NULL	blood	OrganismPart		is exposed to					UV light	PhysicalPhenomenon				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Photopheresis Pheresis treatments involve removing blood from a patient, cycling it through a machine to clean or treat it, and then returning it to the patient. For Sézary Syndrome patients, the blood is exposed to UV light before it is returned to the body. This helps remove affected T-cells from the blood.	topic_ll
76109	20	355712	5	NULL	NULL	0	NULL	statement 19	Process		before returning to					Sézary Syndrome patients	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Photopheresis Pheresis treatments involve removing blood from a patient, cycling it through a machine to clean or treat it, and then returning it to the patient. For Sézary Syndrome patients, the blood is exposed to UV light before it is returned to the body. This helps remove affected T-cells from the blood.	topic_ll
76110	21	355712	5	NULL	NULL	0	NULL	T-cells	Cell	affected	is removed from					blood	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Photopheresis Pheresis treatments involve removing blood from a patient, cycling it through a machine to clean or treat it, and then returning it to the patient. For Sézary Syndrome patients, the blood is exposed to UV light before it is returned to the body. This helps remove affected T-cells from the blood.	topic_ll
76111	22	355712	5	NULL	NULL	NULL	NULL	statement 19	Process		leads to					statement 21	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Photopheresis Pheresis treatments involve removing blood from a patient, cycling it through a machine to clean or treat it, and then returning it to the patient. For Sézary Syndrome patients, the blood is exposed to UV light before it is returned to the body. This helps remove affected T-cells from the blood.	topic_ll
76112	1	355713	5	NULL	NULL	NULL	NULL	Zevalin®	Chemical		is a form of					radioimmunotherapy	MedicalProcedure				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Zevalin® (ibritumomab tiuxetan) is a form of radioimmunotherapy (a radiolabeled monoclonal antibody) indicated for treatment of patients with relapsed or refractory, low grade or follicular B-cell non-Hodgkin's lymphoma (NHL) or for patients with previously untreated follicular NHL who achieve a partial or complete response to first-line chemotherapy.	topic_ll
76113	2	355713	5	NULL	NULL	NULL	NULL	Zevalin®	Chemical		is a type of					radiolabeled monoclonal antibody	GP				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Zevalin® (ibritumomab tiuxetan) is a form of radioimmunotherapy (a radiolabeled monoclonal antibody) indicated for treatment of patients with relapsed or refractory, low grade or follicular B-cell non-Hodgkin's lymphoma (NHL) or for patients with previously untreated follicular NHL who achieve a partial or complete response to first-line chemotherapy.	topic_ll
76114	3	355713	5	NULL	NULL	0	NULL	Zevalin® 	Chemical		is also known as					ibritumomab tiuxetan	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Zevalin® (ibritumomab tiuxetan) is a form of radioimmunotherapy (a radiolabeled monoclonal antibody) indicated for treatment of patients with relapsed or refractory, low grade or follicular B-cell non-Hodgkin's lymphoma (NHL) or for patients with previously untreated follicular NHL who achieve a partial or complete response to first-line chemotherapy.	topic_ll
76115	4	355713	5	NULL	NULL	0	NULL	Zevalin®	Chemical		is used to treat					NHL	MedicalFinding	relapsed or refractory;;low grade or follicular B-cell			NULL		0	NULL	NULL	NULL	NULL	NULL	Zevalin® (ibritumomab tiuxetan) is a form of radioimmunotherapy (a radiolabeled monoclonal antibody) indicated for treatment of patients with relapsed or refractory, low grade or follicular B-cell non-Hodgkin's lymphoma (NHL) or for patients with previously untreated follicular NHL who achieve a partial or complete response to first-line chemotherapy.	topic_ll
76116	5	355713	5	NULL	NULL	0	NULL	NHL	MedicalFinding		is					non-Hodgkin's lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Zevalin® (ibritumomab tiuxetan) is a form of radioimmunotherapy (a radiolabeled monoclonal antibody) indicated for treatment of patients with relapsed or refractory, low grade or follicular B-cell non-Hodgkin's lymphoma (NHL) or for patients with previously untreated follicular NHL who achieve a partial or complete response to first-line chemotherapy.	topic_ll
76117	8	355713	5	NULL	NULL	NULL	NULL	Zevalin®	Chemical		is used to treat					statement 6	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Zevalin® (ibritumomab tiuxetan) is a form of radioimmunotherapy (a radiolabeled monoclonal antibody) indicated for treatment of patients with relapsed or refractory, low grade or follicular B-cell non-Hodgkin's lymphoma (NHL) or for patients with previously untreated follicular NHL who achieve a partial or complete response to first-line chemotherapy.	topic_ll
76118	6	355713	5	NULL	NULL	NULL	NULL	follicular NHL patients	GroupOfPeople	untreated	respond to		partially			first-line chemotherapy	MedicalProcedure				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Zevalin® (ibritumomab tiuxetan) is a form of radioimmunotherapy (a radiolabeled monoclonal antibody) indicated for treatment of patients with relapsed or refractory, low grade or follicular B-cell non-Hodgkin's lymphoma (NHL) or for patients with previously untreated follicular NHL who achieve a partial or complete response to first-line chemotherapy.	topic_ll
76119	7	355713	5	NULL	NULL	0	NULL	follicular NHL patients	GroupOfPeople	untreated	respond to		completely			first-line chemotherapy	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Zevalin® (ibritumomab tiuxetan) is a form of radioimmunotherapy (a radiolabeled monoclonal antibody) indicated for treatment of patients with relapsed or refractory, low grade or follicular B-cell non-Hodgkin's lymphoma (NHL) or for patients with previously untreated follicular NHL who achieve a partial or complete response to first-line chemotherapy.	topic_ll
76120	9	355713	5	NULL	NULL	0	NULL	Zevalin®	Chemical		is used to treat					statement 7	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Zevalin® (ibritumomab tiuxetan) is a form of radioimmunotherapy (a radiolabeled monoclonal antibody) indicated for treatment of patients with relapsed or refractory, low grade or follicular B-cell non-Hodgkin's lymphoma (NHL) or for patients with previously untreated follicular NHL who achieve a partial or complete response to first-line chemotherapy.	topic_ll
76121	1	355714	5	NULL	NULL	0	NULL	lymphoma	MedicalFinding		causes		may			lymph nodes	OrganismPart	swelling of			NULL	neck	0	NULL	NULL	NULL	NULL	NULL	Lymphoma may cause swelling of lymph nodes in the neck, chest, abdomen and on the skin.	topic_ll
76122	2	355714	5	NULL	NULL	0	NULL	lymphoma	MedicalFinding		causes		may			lymph nodes	OrganismPart	swelling of			NULL	chest	0	NULL	NULL	NULL	NULL	NULL	Lymphoma may cause swelling of lymph nodes in the neck, chest, abdomen and on the skin.	topic_ll
76123	3	355714	5	NULL	NULL	0	NULL	lymphoma	MedicalFinding		causes		may			lymph nodes	OrganismPart	swelling of			NULL	abdomen	0	NULL	NULL	NULL	NULL	NULL	Lymphoma may cause swelling of lymph nodes in the neck, chest, abdomen and on the skin.	topic_ll
76124	4	355714	5	NULL	NULL	NULL	NULL	lymphoma	MedicalFinding		causes		may			lymph nodes	OrganismPart	swelling of			NULL	skin	NULL	NULL	NULL	NULL	NULL	NULL	Lymphoma may cause swelling of lymph nodes in the neck, chest, abdomen and on the skin.	topic_ll
76125	1	355715	5	NULL	NULL	0	NULL	lymphoma	MedicalFinding		affects					thymus	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Chest pain Chest pain may occur if the lymphoma affects the thymus	topic_ll
76126	2	355715	5	NULL	NULL	0	NULL	statement 1	Process		causes					Chest pain	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Chest pain Chest pain may occur if the lymphoma affects the thymus	topic_ll
76127	1	355716	5	NULL	NULL	0	NULL	fever	MedicalFinding		recurs					other symptoms	MedicalFinding	 in comjuction with			NULL		0	NULL	NULL	NULL	NULL	NULL	Recurring Fevers Obviously, fever can be a sign of just about anything. When fever recurs for no apparent reason, especially in conjunction with other symptoms, it could be a sign of lymphoma.	topic_ll
76128	2	355716	5	NULL	NULL	0	NULL	statement 1	Process		is a sign of					lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Recurring Fevers Obviously, fever can be a sign of just about anything. When fever recurs for no apparent reason, especially in conjunction with other symptoms, it could be a sign of lymphoma.	topic_ll
76132	1	355717	5	NULL	NULL	0	NULL	pruritis	MedicalFinding		is a synonym of					Itchy skin	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Rashes Itchy skin (pruritis), rashes and lesions can be a sign of lymphoma, particularly cutaneous lymphoma	topic_ll
76133	2	355717	5	NULL	NULL	0	NULL	pruritis	MedicalFinding		is a sign of					cutaneous lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Rashes Itchy skin (pruritis), rashes and lesions can be a sign of lymphoma, particularly cutaneous lymphoma	topic_ll
76134	3	355717	5	NULL	NULL	0	NULL	rashes 	MedicalFinding		is a sign of					cutaneous lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Rashes Itchy skin (pruritis), rashes and lesions can be a sign of lymphoma, particularly cutaneous lymphoma	topic_ll
76135	4	355717	5	NULL	NULL	0	NULL	lesions	MedicalFinding		is a sign of					cutaneous lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Rashes Itchy skin (pruritis), rashes and lesions can be a sign of lymphoma, particularly cutaneous lymphoma	topic_ll
76136	1	355719	5	NULL	NULL	0	NULL	alcohol	Chemical	consumption of	puts stress on					lymphatic system	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Sore lymph nodes after drinking Alchohol consumption puts stress on the lymphatic system which, along with the liver and kidneys, is part of the body's blood cleansing apparatus. If the lymph system is weakened by lymphoma, drinking may cause pain in the affected areas.Lymph nodes are possibly painful after alcohol consumption. 	topic_ll
76137	2	355719	5	NULL	NULL	0	NULL	lymphatic system	OrganismPart		is a part of					blood cleansing apparatus	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Sore lymph nodes after drinking Alchohol consumption puts stress on the lymphatic system which, along with the liver and kidneys, is part of the body's blood cleansing apparatus. If the lymph system is weakened by lymphoma, drinking may cause pain in the affected areas.Lymph nodes are possibly painful after alcohol consumption. 	topic_ll
76138	3	355719	5	NULL	NULL	0	NULL	liver	OrganismPart		is a part of					blood cleansing apparatus	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Sore lymph nodes after drinking Alchohol consumption puts stress on the lymphatic system which, along with the liver and kidneys, is part of the body's blood cleansing apparatus. If the lymph system is weakened by lymphoma, drinking may cause pain in the affected areas.Lymph nodes are possibly painful after alcohol consumption. 	topic_ll
76139	4	355719	5	NULL	NULL	0	NULL	kidneys	OrganismPart		is a part of					blood cleansing apparatus	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Sore lymph nodes after drinking Alchohol consumption puts stress on the lymphatic system which, along with the liver and kidneys, is part of the body's blood cleansing apparatus. If the lymph system is weakened by lymphoma, drinking may cause pain in the affected areas.Lymph nodes are possibly painful after alcohol consumption. 	topic_ll
76140	5	355719	5	NULL	NULL	0	NULL	 lymph system	OrganismPart		is weakened by					lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Sore lymph nodes after drinking Alchohol consumption puts stress on the lymphatic system which, along with the liver and kidneys, is part of the body's blood cleansing apparatus. If the lymph system is weakened by lymphoma, drinking may cause pain in the affected areas.Lymph nodes are possibly painful after alcohol consumption. 	topic_ll
76141	6	355719	5	NULL	NULL	0	NULL	drinking	Process		causes					affected areas	OrganismPart	pain of			NULL		0	NULL	NULL	NULL	NULL	NULL	Sore lymph nodes after drinking Alchohol consumption puts stress on the lymphatic system which, along with the liver and kidneys, is part of the body's blood cleansing apparatus. If the lymph system is weakened by lymphoma, drinking may cause pain in the affected areas.Lymph nodes are possibly painful after alcohol consumption. 	topic_ll
76142	7	355719	5	NULL	NULL	0	NULL	statement 5	Process		leads to					statement 6	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Sore lymph nodes after drinking Alchohol consumption puts stress on the lymphatic system which, along with the liver and kidneys, is part of the body's blood cleansing apparatus. If the lymph system is weakened by lymphoma, drinking may cause pain in the affected areas.Lymph nodes are possibly painful after alcohol consumption. 	topic_ll
76143	8	355719	5	NULL	NULL	NULL	NULL	alcohol	Chemical	consumption of	leads to					painful lymph nodes	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Sore lymph nodes after drinking Alchohol consumption puts stress on the lymphatic system which, along with the liver and kidneys, is part of the body's blood cleansing apparatus. If the lymph system is weakened by lymphoma, drinking may cause pain in the affected areas.Lymph nodes are possibly painful after alcohol consumption. 	topic_ll
76144	1	355720	5	NULL	NULL	0	NULL	AILT	MedicalFinding		is					Angioimmunoblastic T-cell Lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Angioimmunoblastic T-cell Lymphoma (AILT), aka immunoblastic lymphadenopathy, is an aggressive cancer that originates in the T-cells. It accounts for 1% of all Non-Hodgkin’s Lymphomas (NHL) and is found mostly in the elderly. Males have a higher incidence than females.	topic_ll
76145	2	355720	5	NULL	NULL	0	NULL	Angioimmunoblastic T-cell Lymphoma	MedicalFinding		is also known as					immunoblastic lymphadenopathy	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Angioimmunoblastic T-cell Lymphoma (AILT), aka immunoblastic lymphadenopathy, is an aggressive cancer that originates in the T-cells. It accounts for 1% of all Non-Hodgkin’s Lymphomas (NHL) and is found mostly in the elderly. Males have a higher incidence than females.	topic_ll
76146	3	355720	5	NULL	NULL	0	NULL	AILT	MedicalFinding		is a type of					aggressive cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Angioimmunoblastic T-cell Lymphoma (AILT), aka immunoblastic lymphadenopathy, is an aggressive cancer that originates in the T-cells. It accounts for 1% of all Non-Hodgkin’s Lymphomas (NHL) and is found mostly in the elderly. Males have a higher incidence than females.	topic_ll
76147	4	355720	5	NULL	NULL	0	NULL	AILT	MedicalFinding		originates in					T-cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Angioimmunoblastic T-cell Lymphoma (AILT), aka immunoblastic lymphadenopathy, is an aggressive cancer that originates in the T-cells. It accounts for 1% of all Non-Hodgkin’s Lymphomas (NHL) and is found mostly in the elderly. Males have a higher incidence than females.	topic_ll
76148	5	355720	5	NULL	NULL	0	NULL	T-cells	MedicalFinding		found in		mostly			elderly	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Angioimmunoblastic T-cell Lymphoma (AILT), aka immunoblastic lymphadenopathy, is an aggressive cancer that originates in the T-cells. It accounts for 1% of all Non-Hodgkin’s Lymphomas (NHL) and is found mostly in the elderly. Males have a higher incidence than females.	topic_ll
76149	6	355720	5	NULL	NULL	0	NULL	males	GroupOfPeople		higher incidence than					females	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Angioimmunoblastic T-cell Lymphoma (AILT), aka immunoblastic lymphadenopathy, is an aggressive cancer that originates in the T-cells. It accounts for 1% of all Non-Hodgkin’s Lymphomas (NHL) and is found mostly in the elderly. Males have a higher incidence than females.	topic_ll
76150	7	355720	5	NULL	NULL	0	NULL	statement 6	Process		for					AILT	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Angioimmunoblastic T-cell Lymphoma (AILT), aka immunoblastic lymphadenopathy, is an aggressive cancer that originates in the T-cells. It accounts for 1% of all Non-Hodgkin’s Lymphomas (NHL) and is found mostly in the elderly. Males have a higher incidence than females.	topic_ll
76151	1	355721	5	NULL	NULL	0	NULL	Angio	AbstractConcept		refers to					blood	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	"Angio" is a term that refers to the blood vessels. This cancer is marked by the presence of abnormal blood vessels in affected body parts.	topic_ll
76152	2	355721	5	NULL	NULL	0	NULL	blood cancer	MedicalFinding		leads to					blood vessels	OrganismPart	abnormal			NULL	affected body parts	0	NULL	NULL	NULL	NULL	NULL	"Angio" is a term that refers to the blood vessels. This cancer is marked by the presence of abnormal blood vessels in affected body parts.	topic_ll
76153	1	355722	5	NULL	NULL	0	NULL	CHOP 	MedicalProcedure		is a type of					chemotherapy regimen	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	CHOP is one of the most common chemotherapy regimens for treating Non-Hodgkin's lymphoma. Regimen Drugs.	topic_ll
76154	2	355722	5	NULL	NULL	0	NULL	CHOP	MedicalProcedure		is used to treat					Non-Hodgkin's lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	CHOP is one of the most common chemotherapy regimens for treating Non-Hodgkin's lymphoma. Regimen Drugs.	topic_ll
76155	1	355723	5	NULL	NULL	0	NULL	cytoxan	Chemical		is the brand name of					Cyclophosphamide	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The following are the drugs used in the regimen. Select a drug to see a page and pertinent information. * Cyclophosphamide (brand names cytoxan, neosar) * Adriamycin (doxorubicin / hydroxydoxorubicin) * Vincristine (Oncovin) * Prednisone (sometimes called Deltasone or Orasone)	topic_ll
76156	2	355723	5	NULL	NULL	0	NULL	neosar	Chemical		is the brand name of					Cyclophosphamide	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The following are the drugs used in the regimen. Select a drug to see a page and pertinent information. * Cyclophosphamide (brand names cytoxan, neosar) * Adriamycin (doxorubicin / hydroxydoxorubicin) * Vincristine (Oncovin) * Prednisone (sometimes called Deltasone or Orasone)	topic_ll
76160	1	355724	5	NULL	NULL	0	NULL	alopecia	MedicalFinding		is a synonym of					Hair loss	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Hair loss (alopecia) may occur. People have many ways of dealing with hair loss including hats and scarves. 	topic_ll
76161	1	355726	5	NULL	NULL	0	NULL	Non Hodgkin's lymphoma	MedicalFinding		starts in					eye	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Non Hodgkin's lymphoma can start in the eye. It is called ocular lymphoma when it did not start elsewhere including the central nervous system (CNS) (brain etc.) 	topic_ll
76162	2	355726	5	NULL	NULL	0	NULL	statement 1	Process		is called					ocular lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Non Hodgkin's lymphoma can start in the eye. It is called ocular lymphoma when it did not start elsewhere including the central nervous system (CNS) (brain etc.) 	topic_ll
76163	3	355726	5	NULL	NULL	0	NULL	ocular lymphoma	MedicalFinding		does not start in					CNS	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Non Hodgkin's lymphoma can start in the eye. It is called ocular lymphoma when it did not start elsewhere including the central nervous system (CNS) (brain etc.) 	topic_ll
76164	4	355726	5	NULL	NULL	0	NULL	CNS	OrganismPart		is					central nervous system	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Non Hodgkin's lymphoma can start in the eye. It is called ocular lymphoma when it did not start elsewhere including the central nervous system (CNS) (brain etc.) 	topic_ll
76165	1	355731	5	NULL	NULL	0	NULL	hair dye	Chemical		is linked to					lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	There has been a lot of press over the years linking hair dye to lymphoma and other cancers	topic_ll
76167	1	355732	5	NULL	NULL	0	NULL	Henna tattoos	Chemical		is linked to					leukemia	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	Henna tattoos linked to leukaemia risk Researchers believe that certain compounds used with Henna products are causing instances of leukemia. 	topic_ll
76168	1	355733	5	NULL	NULL	0	NULL	Henna tattoos	Chemical		is linked to					leukemia	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	Henna tattoos linked to leukaemia risk 	topic_ll
76169	1	355734	5	NULL	NULL	0	NULL	Benzene	Chemical		used as					solvent	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	They believe that it is not the henna itself that is the problem, but the compounds used as a solvent for the henna powder. Benzene, which is known to cause cancer, is banned for this purpose in many countries, but is still widely employed.	topic_ll
76170	2	355734	5	NULL	NULL	0	NULL	statement 1	Process		is used in					henna powder	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	They believe that it is not the henna itself that is the problem, but the compounds used as a solvent for the henna powder. Benzene, which is known to cause cancer, is banned for this purpose in many countries, but is still widely employed.	topic_ll
76171	3	355734	5	NULL	NULL	0	NULL	Benzene	Chemical		causes					cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	They believe that it is not the henna itself that is the problem, but the compounds used as a solvent for the henna powder. Benzene, which is known to cause cancer, is banned for this purpose in many countries, but is still widely employed.	topic_ll
76173	1	355735	5	NULL	NULL	0	NULL	vitamin K	Chemical	dietary 	is linked to					lymphoma	MedicalFinding	decreased risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary vitamin K linked to decreased lymphoma risk	topic_ll
76175	1	355736	5	NULL	NULL	NULL	NULL	red blood cell transfusion	MedicalProcedure	receiving of	increases					non-Hodgkin's lymphoma	MedicalFinding	risk of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Findings from a meta-study presented at the American Society of Hematology meeting suggest that receiving a red blood cell transfusion increases one's risk of developing a non-Hodgkin's lymphoma. 	topic_ll
76177	1	355737	5	NULL	NULL	0	NULL	red blood cell transfusion	MedicalProcedure		causes					immunosuppression	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Immunosuppression. A red blood cell transfusion causes immunosuppression, which by itself could promote a preexisting NHL to develop.	topic_ll
76180	2	355737	5	NULL	NULL	0	NULL	NHL	MedicalFinding	preexisting	is promoted to					develop	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Immunosuppression. A red blood cell transfusion causes immunosuppression, which by itself could promote a preexisting NHL to develop.	topic_ll
76182	3	355737	5	NULL	NULL	0	NULL	statement 1	Process		leads to					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Immunosuppression. A red blood cell transfusion causes immunosuppression, which by itself could promote a preexisting NHL to develop.	topic_ll
76183	1	355738	5	NULL	NULL	0	NULL	Humira drug	Chemical	consumption of	causes					lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	"Abbott Laboratories was sued by a Texas rheumatoid arthritis sufferer who claims she developed lymphoma after taking its drug Humira in a company-sponsored clinical trial in 2005.	topic_ll
76186	1	355740	5	NULL	NULL	0	NULL	Vitamin C	Chemical	intravenous 	kills		may			lymphoma cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous Vitamin C may Kill Lymphoma Cells	topic_ll
76187	1	355741	5	NULL	NULL	NULL	NULL	malt whisky	Chemical	drinking of	prevents		may			cancer	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Drinking malt whisky may help prevent cancer, a scientific conference has been told. The medicinal properties of antioxidants in red wine are well known, but delegates at a biochemistry conference were told that whisky offered 'even greater health benefits'.	topic_ll
76188	1	355742	5	NULL	NULL	0	NULL	malt whisky	Chemical	drinking of	prevents		may			cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Drinking malt whisky may help prevent cancer, a scientific conference has been told. The medicinal properties of antioxidants in red wine are well known, but delegates at a biochemistry conference were told that whisky offered "even greater health benefits". "However, research has shown that there are even greater health benefits to people who drink single malt whiskies. Why? Single malt whiskies have more ellagic acid than red wine." 	topic_ll
76189	2	355742	5	NULL	NULL	0	NULL	Single malt whiskies	Chemical		contains					ellagic acid	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Drinking malt whisky may help prevent cancer, a scientific conference has been told. The medicinal properties of antioxidants in red wine are well known, but delegates at a biochemistry conference were told that whisky offered "even greater health benefits". "However, research has shown that there are even greater health benefits to people who drink single malt whiskies. Why? Single malt whiskies have more ellagic acid than red wine." 	topic_ll
76190	3	355742	5	NULL	NULL	0	NULL	red wine	Chemical		contains					ellagic acid	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Drinking malt whisky may help prevent cancer, a scientific conference has been told. The medicinal properties of antioxidants in red wine are well known, but delegates at a biochemistry conference were told that whisky offered "even greater health benefits". "However, research has shown that there are even greater health benefits to people who drink single malt whiskies. Why? Single malt whiskies have more ellagic acid than red wine." 	topic_ll
76191	4	355742	5	NULL	NULL	0	NULL	statement 2	Process		is more than					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Drinking malt whisky may help prevent cancer, a scientific conference has been told. The medicinal properties of antioxidants in red wine are well known, but delegates at a biochemistry conference were told that whisky offered "even greater health benefits". "However, research has shown that there are even greater health benefits to people who drink single malt whiskies. Why? Single malt whiskies have more ellagic acid than red wine." 	topic_ll
76193	1	355743	5	NULL	NULL	0	NULL	Single malt whiskies	Chemical		contains					ellagic acid	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	"However, research has shown that there are even greater health benefits to people who drink single malt whiskies. Why? Single malt whiskies have more ellagic acid than red wine." 	topic_ll
76194	2	355743	5	NULL	NULL	0	NULL	red wine	Chemical		contains					ellagic acid	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	"However, research has shown that there are even greater health benefits to people who drink single malt whiskies. Why? Single malt whiskies have more ellagic acid than red wine." 	topic_ll
76195	3	355743	5	NULL	NULL	0	NULL	statement 1	Process		is more than					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	"However, research has shown that there are even greater health benefits to people who drink single malt whiskies. Why? Single malt whiskies have more ellagic acid than red wine." 	topic_ll
76196	1	355744	5	NULL	NULL	0	NULL	autism	MedicalFinding		is associated with					 ITGA4 gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	We recently published evidence of an association between autism and the ITGA4 gene	topic_aut
76197	1	355745	5	NULL	NULL	0	NULL	ITGA3	GP		is not associated with					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	No markers in ITGA3, ITGA6, ITGAV and ITGB3 were found to be associated with autism	topic_aut
76198	2	355745	5	NULL	NULL	0	NULL	ITGA6	GP		is not associated with					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	No markers in ITGA3, ITGA6, ITGAV and ITGB3 were found to be associated with autism	topic_aut
76199	3	355745	5	NULL	NULL	0	NULL	ITGAV	GP		is not associated with					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	No markers in ITGA3, ITGA6, ITGAV and ITGB3 were found to be associated with autism	topic_aut
76200	4	355745	5	NULL	NULL	0	NULL	ITGB3	GP		is not associated with					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	No markers in ITGA3, ITGA6, ITGAV and ITGB3 were found to be associated with autism	topic_aut
76203	1	355746	5	NULL	NULL	NULL	NULL	CD38	GP	low expression of	is associated with					autism	MedicalFinding				NULL	lymphoblastoid cells	NULL	NULL	NULL	NULL	NULL	NULL	Low CD38 expression in lymphoblastoid cells and haplotypes are both associated with autism in a family-based study.	topic_aut
76205	2	355746	5	NULL	NULL	0	NULL	CD38	GP	low expression of	is associated with					autism	MedicalFinding				NULL	haplotypes	0	NULL	NULL	NULL	NULL	NULL	Low CD38 expression in lymphoblastoid cells and haplotypes are both associated with autism in a family-based study.	topic_aut
76207	1	355747	5	NULL	NULL	0	NULL	freeway	GeographicNotProper	living near	is associated with					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Living near a freeway was associated with autism. Examination of associations with measured air pollutants is needed	topic_aut
76208	1	355748	5	NULL	NULL	0	NULL	uridine phosphorylase 2	GP		is associated with					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	uridine phosphorylase 2, with a joint P-value of 2.3E-9, has been previously linked and associated with Autism in independent samples	topic_aut
76210	1	355749	5	NULL	NULL	0	NULL	Calcium channel defects	MedicalFinding		is connected to					ASD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Calcium channel defects have been connected to Autism spectrum disorder (ASD) by Timothy Syndrome, which is Mendelian, and a previous targeted sex-specific association analysis of idiopathic Autism	topic_aut
76211	2	355749	5	NULL	NULL	0	NULL	ASD	MedicalFinding		is					Autism spectrum disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Calcium channel defects have been connected to Autism spectrum disorder (ASD) by Timothy Syndrome, which is Mendelian, and a previous targeted sex-specific association analysis of idiopathic Autism	topic_aut
76225	3	355749	5	NULL	NULL	0	NULL	Timothy Syndrome	MedicalFinding		plays a role in					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Calcium channel defects have been connected to Autism spectrum disorder (ASD) by Timothy Syndrome, which is Mendelian, and a previous targeted sex-specific association analysis of idiopathic Autism	topic_aut
76276	1	355750	5	NULL	NULL	NULL	NULL	autistic children	GroupOfPeople		more likely to have					mitochondrial dysfunction	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this exploratory study, children with autism were more likely to have mitochondrial dysfunction, mtDNA overreplication, and mtDNA deletions than typically developing children	topic_aut
76277	2	355750	5	NULL	NULL	NULL	NULL	autistic children	GroupOfPeople		more likely to have					mtDNA overreplication	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this exploratory study, children with autism were more likely to have mitochondrial dysfunction, mtDNA overreplication, and mtDNA deletions than typically developing children	topic_aut
76278	3	355750	5	NULL	NULL	NULL	NULL	autistic children	GroupOfPeople		more likely to have					mtDNA deletions	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this exploratory study, children with autism were more likely to have mitochondrial dysfunction, mtDNA overreplication, and mtDNA deletions than typically developing children	topic_aut
76279	1	355751	5	NULL	NULL	NULL	NULL	ITGB3	GP		is					integrin-beta 3 gene	GP				NULL		NULL	NULL	NULL	NULL	NULL	NULL	The integrin-β 3 gene (ITGB3), located on human chromosome 17q21.3, was previously identified as a quantitative trait locus (QTL) for 5-HT blood levels and has been implicated as a candidate gene for autism spectrum disorder (ASD)	topic_aut
76280	2	355751	5	NULL	NULL	0	NULL	ITGB3	GP		is located on					chromosome 17q21.3	Chromosome	human			NULL		0	NULL	NULL	NULL	NULL	NULL	The integrin-β 3 gene (ITGB3), located on human chromosome 17q21.3, was previously identified as a quantitative trait locus (QTL) for 5-HT blood levels and has been implicated as a candidate gene for autism spectrum disorder (ASD)	topic_aut
76281	3	355751	5	NULL	NULL	0	NULL	ITGB3	GP		is a type of					QTL	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	The integrin-β 3 gene (ITGB3), located on human chromosome 17q21.3, was previously identified as a quantitative trait locus (QTL) for 5-HT blood levels and has been implicated as a candidate gene for autism spectrum disorder (ASD)	topic_aut
76282	4	355751	5	NULL	NULL	0	NULL	QTL	Chromosome		is					quantitative trait locus	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	The integrin-β 3 gene (ITGB3), located on human chromosome 17q21.3, was previously identified as a quantitative trait locus (QTL) for 5-HT blood levels and has been implicated as a candidate gene for autism spectrum disorder (ASD)	topic_aut
76283	5	355751	5	NULL	NULL	0	NULL	statement 4	Process		for					5-HT	GP	levels of;;blood			NULL		0	NULL	NULL	NULL	NULL	NULL	The integrin-β 3 gene (ITGB3), located on human chromosome 17q21.3, was previously identified as a quantitative trait locus (QTL) for 5-HT blood levels and has been implicated as a candidate gene for autism spectrum disorder (ASD)	topic_aut
76284	6	355751	5	NULL	NULL	0	NULL	ITGB3	GP		is a candidate gene for					ASD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The integrin-β 3 gene (ITGB3), located on human chromosome 17q21.3, was previously identified as a quantitative trait locus (QTL) for 5-HT blood levels and has been implicated as a candidate gene for autism spectrum disorder (ASD)	topic_aut
76285	7	355751	5	NULL	NULL	0	NULL	ASD	MedicalFinding		is					autism spectrum disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The integrin-β 3 gene (ITGB3), located on human chromosome 17q21.3, was previously identified as a quantitative trait locus (QTL) for 5-HT blood levels and has been implicated as a candidate gene for autism spectrum disorder (ASD)	topic_aut
76286	1	355752	5	NULL	NULL	0	NULL	RTT	MedicalFinding		is					Rett syndrome	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Rett syndrome (RTT) as an ASD genetic model	topic_aut
76287	2	355752	5	NULL	NULL	0	NULL	Rett syndrome	MedicalFinding		is a genetic model of					ASD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Rett syndrome (RTT) as an ASD genetic model	topic_aut
76288	1	355754	5	NULL	NULL	0	NULL	early alterations	Process		is present in					RTT neurons	OrganismPart	developing;;human			NULL		0	NULL	NULL	NULL	NULL	NULL	Our data uncovered early alterations in developing human RTT neurons	topic_aut
76289	1	355755	5	NULL	NULL	0	NULL	MECP2 gene	GP		is a type of					X-linked gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the X-linked MECP2 gene, which encodes the transcriptional regulator methyl-CpG-binding protein 2 (MeCP2), cause Rett syndrome and several neurodevelopmental disorders including cognitive disorders, autism, juvenile-onset schizophrenia and encephalopathy with early lethality	topic_aut
76290	2	355755	5	NULL	NULL	0	NULL	MECP2 gene	GP		encodes					methyl-CpG-binding protein 2	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the X-linked MECP2 gene, which encodes the transcriptional regulator methyl-CpG-binding protein 2 (MeCP2), cause Rett syndrome and several neurodevelopmental disorders including cognitive disorders, autism, juvenile-onset schizophrenia and encephalopathy with early lethality	topic_aut
76291	3	355755	5	NULL	NULL	0	NULL	methyl-CpG-binding protein 2	GP		is					MeCP2	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the X-linked MECP2 gene, which encodes the transcriptional regulator methyl-CpG-binding protein 2 (MeCP2), cause Rett syndrome and several neurodevelopmental disorders including cognitive disorders, autism, juvenile-onset schizophrenia and encephalopathy with early lethality	topic_aut
76292	4	355755	5	NULL	NULL	0	NULL	MeCP2	GP		is a type of					transcriptional regulator	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the X-linked MECP2 gene, which encodes the transcriptional regulator methyl-CpG-binding protein 2 (MeCP2), cause Rett syndrome and several neurodevelopmental disorders including cognitive disorders, autism, juvenile-onset schizophrenia and encephalopathy with early lethality	topic_aut
76293	5	355755	5	NULL	NULL	0	NULL	MECP2 gene	GP	mutation of	cause					Rett syndrome	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the X-linked MECP2 gene, which encodes the transcriptional regulator methyl-CpG-binding protein 2 (MeCP2), cause Rett syndrome and several neurodevelopmental disorders including cognitive disorders, autism, juvenile-onset schizophrenia and encephalopathy with early lethality	topic_aut
76294	6	355755	5	NULL	NULL	0	NULL	MECP2 gene	GP		cause					cognitive disorders	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the X-linked MECP2 gene, which encodes the transcriptional regulator methyl-CpG-binding protein 2 (MeCP2), cause Rett syndrome and several neurodevelopmental disorders including cognitive disorders, autism, juvenile-onset schizophrenia and encephalopathy with early lethality	topic_aut
76295	7	355755	5	NULL	NULL	0	NULL	MECP2 gene	GP	mutation of	cause					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the X-linked MECP2 gene, which encodes the transcriptional regulator methyl-CpG-binding protein 2 (MeCP2), cause Rett syndrome and several neurodevelopmental disorders including cognitive disorders, autism, juvenile-onset schizophrenia and encephalopathy with early lethality	topic_aut
76296	8	355755	5	NULL	NULL	0	NULL	MECP2 gene	GP	mutation of	cause					juvenile-onset schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the X-linked MECP2 gene, which encodes the transcriptional regulator methyl-CpG-binding protein 2 (MeCP2), cause Rett syndrome and several neurodevelopmental disorders including cognitive disorders, autism, juvenile-onset schizophrenia and encephalopathy with early lethality	topic_aut
76297	9	355755	5	NULL	NULL	0	NULL	MECP2 gene	GP	mutation of	cause					encephalopathy	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the X-linked MECP2 gene, which encodes the transcriptional regulator methyl-CpG-binding protein 2 (MeCP2), cause Rett syndrome and several neurodevelopmental disorders including cognitive disorders, autism, juvenile-onset schizophrenia and encephalopathy with early lethality	topic_aut
76298	10	355755	5	NULL	NULL	0	NULL	cognitive disorders	MedicalFinding		is a type of					neurodevelopmental disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the X-linked MECP2 gene, which encodes the transcriptional regulator methyl-CpG-binding protein 2 (MeCP2), cause Rett syndrome and several neurodevelopmental disorders including cognitive disorders, autism, juvenile-onset schizophrenia and encephalopathy with early lethality	topic_aut
76299	11	355755	5	NULL	NULL	0	NULL	autism	MedicalFinding		is a type of					neurodevelopmental disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the X-linked MECP2 gene, which encodes the transcriptional regulator methyl-CpG-binding protein 2 (MeCP2), cause Rett syndrome and several neurodevelopmental disorders including cognitive disorders, autism, juvenile-onset schizophrenia and encephalopathy with early lethality	topic_aut
76300	12	355755	5	NULL	NULL	0	NULL	juvenile-onset schizophrenia	MedicalFinding		is a type of					neurodevelopmental disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the X-linked MECP2 gene, which encodes the transcriptional regulator methyl-CpG-binding protein 2 (MeCP2), cause Rett syndrome and several neurodevelopmental disorders including cognitive disorders, autism, juvenile-onset schizophrenia and encephalopathy with early lethality	topic_aut
76301	13	355755	5	NULL	NULL	0	NULL	encephalopathy	MedicalFinding		is a type of					neurodevelopmental disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the X-linked MECP2 gene, which encodes the transcriptional regulator methyl-CpG-binding protein 2 (MeCP2), cause Rett syndrome and several neurodevelopmental disorders including cognitive disorders, autism, juvenile-onset schizophrenia and encephalopathy with early lethality	topic_aut
76535	1	355756	11	NULL	NULL	0	NULL	Empirical therapy	MedicalProcedure		 is recommended for					Beta-hemolytic streptococci	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Empirical therapy for Beta-hemolytic streptococci is recommended. Empirical coverage for CA-MRSA is recommended in patients who do not respond to Beta-lactam therapy and may be considered in those with systemic toxicity. 	topic_mrs
76536	2	355756	11	NULL	NULL	0	NULL	Empirical coverage	MedicalProcedure		is recommended for					CA-MRSA	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Empirical therapy for Beta-hemolytic streptococci is recommended. Empirical coverage for CA-MRSA is recommended in patients who do not respond to Beta-lactam therapy and may be considered in those with systemic toxicity. 	topic_mrs
76537	1	355757	11	NULL	NULL	NULL	NULL	Nonpurulent cellulitis	MedicalFinding		have no					purulent drainage	BiologicalProcess				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nonpurulent cellulitis is defined as cellulitis with no purulent drainage or exudate and no associated abscess.	topic_mrs
76538	2	355757	11	NULL	NULL	NULL	NULL	Nonpurulent cellulitis	MedicalFinding		have no					exudate	BiologicalProcess				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nonpurulent cellulitis is defined as cellulitis with no purulent drainage or exudate and no associated abscess.	topic_mrs
76539	3	355757	11	NULL	NULL	0	NULL	Nonpurulent cellulitis	MedicalFinding		have no					abscess	MedicalFinding	associated			NULL		0	NULL	NULL	NULL	NULL	NULL	Nonpurulent cellulitis is defined as cellulitis with no purulent drainage or exudate and no associated abscess.	topic_mrs
77235	1	355758	11	NULL	NULL	NULL	NULL	cellulitis	MedicalFinding		is associated with					purulent drainage	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Purulent cellulitis is cellulitis associated with purulent drainage or exudate in the absence of a drainable abscess	topic_mrs
77236	2	355758	11	NULL	NULL	0	NULL	statement 1	Process		is known as					Purulent cellulitis	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Purulent cellulitis is cellulitis associated with purulent drainage or exudate in the absence of a drainable abscess	topic_mrs
77237	3	355758	11	NULL	NULL	0	NULL	exudate	MedicalFinding		in the absence of					abscess	MedicalFinding	drainable			NULL		0	NULL	NULL	NULL	NULL	NULL	Purulent cellulitis is cellulitis associated with purulent drainage or exudate in the absence of a drainable abscess	topic_mrs
77238	4	355758	11	NULL	NULL	0	NULL	statement 3	Process		is known as					Purulent cellulitis	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Purulent cellulitis is cellulitis associated with purulent drainage or exudate in the absence of a drainable abscess	topic_mrs
76239	1	355759	11	NULL	NULL	0	NULL	Telavancin	Chemical		is a type of 					bactericidal lipoglycopeptide	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Telavancin (trade name Vibativ) is a bactericidal lipoglycopeptide for use in MRSA or other Gram-positive infections. Telavancin is a synthetic derivative of vancomycin.	topic_mrs
76240	2	355759	11	NULL	NULL	0	NULL	Telavancin	Chemical		is a synonym of					Vibativ	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Telavancin (trade name Vibativ) is a bactericidal lipoglycopeptide for use in MRSA or other Gram-positive infections. Telavancin is a synthetic derivative of vancomycin.	topic_mrs
76241	3	355759	11	NULL	NULL	NULL	NULL	Telavancin	Chemical		used in					 infections	BiologicalProcess	MRSA ;; Gram-positive			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Telavancin (trade name Vibativ) is a bactericidal lipoglycopeptide for use in MRSA or other Gram-positive infections. Telavancin is a synthetic derivative of vancomycin.	topic_mrs
76242	4	355759	11	NULL	NULL	NULL	NULL	Telavancin	Chemical		is a derivative of		synthetic 			vancomycin	Chemical				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Telavancin (trade name Vibativ) is a bactericidal lipoglycopeptide for use in MRSA or other Gram-positive infections. Telavancin is a synthetic derivative of vancomycin.	topic_mrs
76540	1	355760	11	NULL	NULL	0	NULL	lipoglycopeptides	Chemical		are a class of 					antibiotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	lipoglycopeptides are a class of antibiotic that have lipophilic side-chains linked to glycopeptides. The class includes oritavancin, telavancin and dalbavancin.	topic_mrs
76541	2	355760	11	NULL	NULL	0	NULL	lipoglycopeptides	Chemical		includes					oritavancin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	lipoglycopeptides are a class of antibiotic that have lipophilic side-chains linked to glycopeptides. The class includes oritavancin, telavancin and dalbavancin.	topic_mrs
76542	3	355760	11	NULL	NULL	0	NULL	lipoglycopeptide	Chemical		includes					telavancin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	lipoglycopeptides are a class of antibiotic that have lipophilic side-chains linked to glycopeptides. The class includes oritavancin, telavancin and dalbavancin.	topic_mrs
76543	4	355760	11	NULL	NULL	0	NULL	lipoglycopeptides	Chemical		includes					dalbavancin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	lipoglycopeptides are a class of antibiotic that have lipophilic side-chains linked to glycopeptides. The class includes oritavancin, telavancin and dalbavancin.	topic_mrs
76243	1	355761	11	NULL	NULL	0	NULL	Telavancin	Chemical		approved for		FDA			 cSSTI	MedicalFinding	in adults			NULL		0	NULL	NULL	NULL	NULL	NULL	Telavancin is FDA-approved for cSSTI in adults	topic_mrs
76244	1	355762	11	NULL	NULL	0	NULL	Tetracycline	Chemical		is a type of 					polyketide antibiotic	Chemical	broad-spectrum			NULL		0	NULL	NULL	NULL	NULL	NULL	Tetracycline is a broad-spectrum polyketide antibiotic produced by the Streptomyces genus of Actinobacteria, indicated for use against many bacterial infections. 	topic_mrs
76245	2	355762	11	NULL	NULL	0	NULL	Streptomyces	Organism		is a genus of					Actinobacteria	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Tetracycline is a broad-spectrum polyketide antibiotic produced by the Streptomyces genus of Actinobacteria, indicated for use against many bacterial infections. 	topic_mrs
76246	3	355762	11	NULL	NULL	0	NULL	Tetracycline	Chemical		is produced by 					Streptomyces	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Tetracycline is a broad-spectrum polyketide antibiotic produced by the Streptomyces genus of Actinobacteria, indicated for use against many bacterial infections. 	topic_mrs
76247	4	355762	11	NULL	NULL	NULL	NULL	Tetracycline	Chemical		used against		can be			infections	BiologicalProcess	 bacterial 			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Tetracycline is a broad-spectrum polyketide antibiotic produced by the Streptomyces genus of Actinobacteria, indicated for use against many bacterial infections. 	topic_mrs
76935	1	355763	11	NULL	NULL	0	NULL	S. aureus	Organism		causes					SSTI	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Doxycycline is FDA-approved for the treatment of SSTI due to S. aureus, although not speciﬁcally for those caused by MRSA	topic_mrs
76936	2	355763	11	NULL	NULL	0	NULL	MRSA	Organism		causes					SSTI	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Doxycycline is FDA-approved for the treatment of SSTI due to S. aureus, although not speciﬁcally for those caused by MRSA	topic_mrs
76937	3	355763	11	NULL	NULL	0	NULL	Doxycycline	Chemical		treats					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Doxycycline is FDA-approved for the treatment of SSTI due to S. aureus, although not speciﬁcally for those caused by MRSA	topic_mrs
76938	1	355764	11	NULL	NULL	0	NULL	murein	Chemical		is a type of 					polymer	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	murein is a polymer consisting of sugars and amino acids that forms a mesh-like layer outside the plasma membrane of bacteria 	topic_mrs
76939	2	355764	11	NULL	NULL	0	NULL	murein	Chemical		consisting of					sugars	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	murein is a polymer consisting of sugars and amino acids that forms a mesh-like layer outside the plasma membrane of bacteria 	topic_mrs
76940	3	355764	11	NULL	NULL	0	NULL	murein	Chemical		consisting of					 amino acids	amino acid				NULL		0	NULL	NULL	NULL	NULL	NULL	murein is a polymer consisting of sugars and amino acids that forms a mesh-like layer outside the plasma membrane of bacteria 	topic_mrs
76941	4	355764	11	NULL	NULL	0	NULL	statement 2	Process		occurs along with					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	murein is a polymer consisting of sugars and amino acids that forms a mesh-like layer outside the plasma membrane of bacteria 	topic_mrs
76942	5	355764	11	NULL	NULL	0	NULL	murein	Chemical		forms a					mesh-like layer	CellComponent	outside the plasma membrane			NULL	 bacteria	0	NULL	NULL	NULL	NULL	NULL	murein is a polymer consisting of sugars and amino acids that forms a mesh-like layer outside the plasma membrane of bacteria 	topic_mrs
76943	1	355765	11	NULL	NULL	NULL	NULL	Penicillin	Chemical		impaires					cell wall synthesis	BiologicalProcess	bacteria			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Penicillin kills bacteria by interfering with the ability to synthesize cell wall.	topic_mrs
76944	2	355765	11	NULL	NULL	0	NULL	statement 1	Process		kills					bacteria	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Penicillin kills bacteria by interfering with the ability to synthesize cell wall.	topic_mrs
76945	1	355766	11	NULL	NULL	0	NULL	MRSA	Organism		is a strain of					Staphylococcus aureus bacteria	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA is, by definition, any strain of Staphylococcus aureus bacteria that has developed resistance to beta-lactam antibiotics which include the penicillins 	topic_mrs
76946	2	355766	11	NULL	NULL	0	NULL	MRSA	Organism		has resistance to					beta-lactam antibiotics	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA is, by definition, any strain of Staphylococcus aureus bacteria that has developed resistance to beta-lactam antibiotics which include the penicillins 	topic_mrs
76947	3	355766	11	NULL	NULL	0	NULL	 penicillins	Chemical		is a type of 					 beta-lactam antibiotics	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA is, by definition, any strain of Staphylococcus aureus bacteria that has developed resistance to beta-lactam antibiotics which include the penicillins 	topic_mrs
76948	4	355766	11	NULL	NULL	0	NULL	MRSA	Organism		has resistance to					penicillins	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA is, by definition, any strain of Staphylococcus aureus bacteria that has developed resistance to beta-lactam antibiotics which include the penicillins 	topic_mrs
76949	1	355767	11	NULL	NULL	NULL	NULL	 community-associated MRSA	Organism		causes		possibly			 infections	MedicalFinding	skin;; soft tissue			NULL		NULL	NULL	NULL	NULL	NULL	NULL	About 75 percent of community-associated (CA-) MRSA infections are localized to skin and soft tissue and usually can be treated effectively. However, some CA-MRSA strains display enhanced virulence, spreading more rapidly and causing illness much more severe than traditional healthcare-associated (HA-) MRSA infections, and they can affect vital organs and lead to widespread infection	topic_mrs
76950	2	355767	11	NULL	NULL	0	NULL	CA-MRSA	Organism		is					community-associated MRSA	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	About 75 percent of community-associated (CA-) MRSA infections are localized to skin and soft tissue and usually can be treated effectively. However, some CA-MRSA strains display enhanced virulence, spreading more rapidly and causing illness much more severe than traditional healthcare-associated (HA-) MRSA infections, and they can affect vital organs and lead to widespread infection	topic_mrs
76951	3	355767	11	NULL	NULL	NULL	NULL	CA-MRSA	Organism		causes		can			widespread infection	MedicalFinding	vital organs			NULL		NULL	NULL	NULL	NULL	NULL	NULL	About 75 percent of community-associated (CA-) MRSA infections are localized to skin and soft tissue and usually can be treated effectively. However, some CA-MRSA strains display enhanced virulence, spreading more rapidly and causing illness much more severe than traditional healthcare-associated (HA-) MRSA infections, and they can affect vital organs and lead to widespread infection	topic_mrs
76952	1	355768	11	NULL	NULL	0	NULL	PVL	Chemical		is a type of 					CA-MRSA toxin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	and they can affect vital organs and lead to widespread infection (sepsis), toxic shock syndrome and necrotizing ('flesh-eating') pneumonia. This is thought to be due to toxins carried by CA-MRSA strains, such as PVL and PSM	topic_mrs
76953	2	355768	11	NULL	NULL	0	NULL	PSM	Chemical		is a type of 					CA-MRSA toxin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	and they can affect vital organs and lead to widespread infection (sepsis), toxic shock syndrome and necrotizing ('flesh-eating') pneumonia. This is thought to be due to toxins carried by CA-MRSA strains, such as PVL and PSM	topic_mrs
76954	3	355768	11	NULL	NULL	0	NULL	CA-MRSA strain	Organism		produces					toxins	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	and they can affect vital organs and lead to widespread infection (sepsis), toxic shock syndrome and necrotizing ('flesh-eating') pneumonia. This is thought to be due to toxins carried by CA-MRSA strains, such as PVL and PSM	topic_mrs
76955	4	355768	11	NULL	NULL	NULL	NULL	CA-MRSA strain	Organism		causes					widespread infection	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	and they can affect vital organs and lead to widespread infection (sepsis), toxic shock syndrome and necrotizing ('flesh-eating') pneumonia. This is thought to be due to toxins carried by CA-MRSA strains, such as PVL and PSM	topic_mrs
76956	5	355768	11	NULL	NULL	0	NULL	CA-MRSA strain	Organism		causes					toxic shock syndrome	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	and they can affect vital organs and lead to widespread infection (sepsis), toxic shock syndrome and necrotizing ('flesh-eating') pneumonia. This is thought to be due to toxins carried by CA-MRSA strains, such as PVL and PSM	topic_mrs
76957	6	355768	11	NULL	NULL	0	NULL	CA-MRSA strain	Organism		causes					necrotizing pneumonia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	and they can affect vital organs and lead to widespread infection (sepsis), toxic shock syndrome and necrotizing ('flesh-eating') pneumonia. This is thought to be due to toxins carried by CA-MRSA strains, such as PVL and PSM	topic_mrs
76958	7	355768	11	NULL	NULL	NULL	NULL	sepsis	MedicalFinding		is also known as					infection	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	and they can affect vital organs and lead to widespread infection (sepsis), toxic shock syndrome and necrotizing ('flesh-eating') pneumonia. This is thought to be due to toxins carried by CA-MRSA strains, such as PVL and PSM	topic_mrs
76979	1	355769	11	NULL	NULL	0	NULL	Bacteria	Organism		express					lipopeptide	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	A lipopeptide is a molecule consisting of a lipid connected to a peptide. Bacteria express these molecules. They are bound by TLR 1, and other, Toll-like receptors. Certain lipopeptides are used as antibiotics.	topic_mrs
76980	2	355769	11	NULL	NULL	0	NULL	TLR 1	GP		is a type of 					Toll-like receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	A lipopeptide is a molecule consisting of a lipid connected to a peptide. Bacteria express these molecules. They are bound by TLR 1, and other, Toll-like receptors. Certain lipopeptides are used as antibiotics.	topic_mrs
76981	3	355769	11	NULL	NULL	0	NULL	 lipopeptide	Chemical		bounds by					Toll-like receptors	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	A lipopeptide is a molecule consisting of a lipid connected to a peptide. Bacteria express these molecules. They are bound by TLR 1, and other, Toll-like receptors. Certain lipopeptides are used as antibiotics.	topic_mrs
76982	4	355769	11	NULL	NULL	0	NULL	 lipopeptide	Chemical		bounds by					TLR 1	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	A lipopeptide is a molecule consisting of a lipid connected to a peptide. Bacteria express these molecules. They are bound by TLR 1, and other, Toll-like receptors. Certain lipopeptides are used as antibiotics.	topic_mrs
76983	5	355769	11	NULL	NULL	0	NULL	lipopeptides	Chemical		are used as		possibly			antibiotics	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	A lipopeptide is a molecule consisting of a lipid connected to a peptide. Bacteria express these molecules. They are bound by TLR 1, and other, Toll-like receptors. Certain lipopeptides are used as antibiotics.	topic_mrs
76985	1	355770	11	NULL	NULL	NULL	NULL	Endocarditis	MedicalFinding		is a type of 					inflammation	MedicalFinding	endocardium;;heart valves			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Endocarditis is an inflammation of the inner layer of the heart, the endocardium. It usually involves the heart valves	topic_mrs
76986	2	355770	11	NULL	NULL	0	NULL	endocardium	OrganismPart		is a type of 					inner layer of the heart	Organism part				NULL		0	NULL	NULL	NULL	NULL	NULL	Endocarditis is an inflammation of the inner layer of the heart, the endocardium. It usually involves the heart valves	topic_mrs
76987	1	355771	11	NULL	NULL	0	NULL	ORSA	Organism		is					Oxacillin Resistant Staph aureus	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	ORSA stands for Oxacillin Resistant Staph aureus. MRSA stands for Methicillin Resistant Staph aureus. ORSA and MRSA are different names for the same bacteria. Oxacillin and Methicillin are in the penicillin drug family, and some strains of Staph have become resistant to both of these antibiotics as well as other related antibiotics. Other drugs can be used to treat infections caused by this bacteria.	topic_mrs
76988	2	355771	11	NULL	NULL	0	NULL	MRSA	Organism		is					Methicillin Resistant Staph aureus	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	ORSA stands for Oxacillin Resistant Staph aureus. MRSA stands for Methicillin Resistant Staph aureus. ORSA and MRSA are different names for the same bacteria. Oxacillin and Methicillin are in the penicillin drug family, and some strains of Staph have become resistant to both of these antibiotics as well as other related antibiotics. Other drugs can be used to treat infections caused by this bacteria.	topic_mrs
76989	3	355771	11	NULL	NULL	0	NULL	ORSA	Organism		is also known as					 MRSA 	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	ORSA stands for Oxacillin Resistant Staph aureus. MRSA stands for Methicillin Resistant Staph aureus. ORSA and MRSA are different names for the same bacteria. Oxacillin and Methicillin are in the penicillin drug family, and some strains of Staph have become resistant to both of these antibiotics as well as other related antibiotics. Other drugs can be used to treat infections caused by this bacteria.	topic_mrs
76990	4	355771	11	NULL	NULL	0	NULL	Oxacillin	Chemical		is a type of 					penicillin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	ORSA stands for Oxacillin Resistant Staph aureus. MRSA stands for Methicillin Resistant Staph aureus. ORSA and MRSA are different names for the same bacteria. Oxacillin and Methicillin are in the penicillin drug family, and some strains of Staph have become resistant to both of these antibiotics as well as other related antibiotics. Other drugs can be used to treat infections caused by this bacteria.	topic_mrs
76991	5	355771	11	NULL	NULL	0	NULL	Methicillin	Chemical		is a type of 					penicillin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	ORSA stands for Oxacillin Resistant Staph aureus. MRSA stands for Methicillin Resistant Staph aureus. ORSA and MRSA are different names for the same bacteria. Oxacillin and Methicillin are in the penicillin drug family, and some strains of Staph have become resistant to both of these antibiotics as well as other related antibiotics. Other drugs can be used to treat infections caused by this bacteria.	topic_mrs
76992	6	355771	11	NULL	NULL	0	NULL	Staph strains	Organism		become resistant to		may			Oxacillin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	ORSA stands for Oxacillin Resistant Staph aureus. MRSA stands for Methicillin Resistant Staph aureus. ORSA and MRSA are different names for the same bacteria. Oxacillin and Methicillin are in the penicillin drug family, and some strains of Staph have become resistant to both of these antibiotics as well as other related antibiotics. Other drugs can be used to treat infections caused by this bacteria.	topic_mrs
76993	7	355771	11	NULL	NULL	0	NULL	Staph strains	Organism		become resistant to		may			methicillin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	ORSA stands for Oxacillin Resistant Staph aureus. MRSA stands for Methicillin Resistant Staph aureus. ORSA and MRSA are different names for the same bacteria. Oxacillin and Methicillin are in the penicillin drug family, and some strains of Staph have become resistant to both of these antibiotics as well as other related antibiotics. Other drugs can be used to treat infections caused by this bacteria.	topic_mrs
76994	1	355772	11	NULL	NULL	0	NULL	clonal complex 398	Organism		is a subtype of					methicillin-resistant Staphylococcus aureus	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	n emerging subtype of methicillin-resistant Staphylococcus aureus (MRSA), clonal complex (CC) 398, is associated with animals, particularly pigs.	topic_mrs
76995	2	355772	11	NULL	NULL	0	NULL	methicillin-resistant Staphylococcus aureus	Organism		is					MRSA	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	n emerging subtype of methicillin-resistant Staphylococcus aureus (MRSA), clonal complex (CC) 398, is associated with animals, particularly pigs.	topic_mrs
76996	3	355772	11	NULL	NULL	0	NULL	clonal complex 398	Organism		is associated with					 pigs	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	n emerging subtype of methicillin-resistant Staphylococcus aureus (MRSA), clonal complex (CC) 398, is associated with animals, particularly pigs.	topic_mrs
76997	4	355772	11	NULL	NULL	0	NULL	clonal complex 398	Organism		 is associated with					animals	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	n emerging subtype of methicillin-resistant Staphylococcus aureus (MRSA), clonal complex (CC) 398, is associated with animals, particularly pigs.	topic_mrs
76302	1	355774	5	NULL	NULL	0	NULL	BCL6	GP		is a type of					oncogene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Here's what we know: The oncogene known as BCL6 is generally associated with diffuse large B-cell lymphoma (DLBCL).	topic_ll
76303	2	355774	5	NULL	NULL	0	NULL	BCL6	GP		is associated with					DLBCL	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Here's what we know: The oncogene known as BCL6 is generally associated with diffuse large B-cell lymphoma (DLBCL).	topic_ll
76304	3	355774	5	NULL	NULL	0	NULL	DLBCL	MedicalFinding		is					diffuse large B-cell lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Here's what we know: The oncogene known as BCL6 is generally associated with diffuse large B-cell lymphoma (DLBCL).	topic_ll
76305	1	355775	5	NULL	NULL	0	NULL	79-6	Chemical		is an inhibitor of					BCL6	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	So researchers have gone looking for the right BCL6 inhibitor, and they may have found it in a compound known as 79-6, which has proven effective in killing the DLBCL cell lines.	topic_ll
76306	2	355775	5	NULL	NULL	0	NULL	79-6	Chemical		kills		effectively			DLBCL cell lines	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	So researchers have gone looking for the right BCL6 inhibitor, and they may have found it in a compound known as 79-6, which has proven effective in killing the DLBCL cell lines.	topic_ll
76307	1	355778	5	NULL	NULL	0	NULL	BEACOPP regimen	MedicalProcedure		is used to treat					HL	MedicalFinding	late-stage;;unfavorable			NULL		0	NULL	NULL	NULL	NULL	NULL	The BEACOPP regimen was established by the GHSG in 1989 for the treatment of late-stage, unfavorable HL. 	topic_ll
76308	2	355778	5	NULL	NULL	0	NULL	BEACOPP regimen	MedicalProcedure		established by					GHSG	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	The BEACOPP regimen was established by the GHSG in 1989 for the treatment of late-stage, unfavorable HL. 	topic_ll
76309	1	355779	5	NULL	NULL	0	NULL	Pralatrexate	Chemical		is a type of					orphan drug	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Pralatrexate given orphan drug status for CTCL in Europe	topic_ll
76310	2	355779	5	NULL	NULL	0	NULL	Pralatrexate	Chemical		is used to treat					CTCL	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Pralatrexate given orphan drug status for CTCL in Europe	topic_ll
77045	1	355782	11	NULL	NULL	0	NULL	Silver	Chemical		purify					water	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Silver has been used since antiquity to purify water.  While silver's importance as a bactericide has only been documented since the late 1800s, its use in purification has been known throughout the ages.	topic_mrs
77046	2	355782	11	NULL	NULL	0	NULL	Silver	Chemical		is a type of 					bactericide	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Silver has been used since antiquity to purify water.  While silver's importance as a bactericide has only been documented since the late 1800s, its use in purification has been known throughout the ages.	topic_mrs
77047	1	355783	11	NULL	NULL	0	NULL	Colloidal Silver	Chemical		kill					organisms	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Colloidal Silver is thought to kill an average of 650 different organisms, compared to the 6 of a standard antibiotic.  It is safe for adults, children, animals and pregnant and nursing women. It can be applied topically and used internally and has no reaction with other medications.	topic_mrs
77125	2	355783	11	NULL	NULL	0	NULL	Colloidal Silver\t	Chemical		has no reaction with					medications	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Colloidal Silver is thought to kill an average of 650 different organisms, compared to the 6 of a standard antibiotic.  It is safe for adults, children, animals and pregnant and nursing women. It can be applied topically and used internally and has no reaction with other medications.	topic_mrs
77126	3	355783	11	NULL	NULL	0	NULL	Colloidal Silver	Chemical		can be applied 					topically	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Colloidal Silver is thought to kill an average of 650 different organisms, compared to the 6 of a standard antibiotic.  It is safe for adults, children, animals and pregnant and nursing women. It can be applied topically and used internally and has no reaction with other medications.	topic_mrs
77127	4	355783	11	NULL	NULL	0	NULL	Colloidal Silver	Chemical		can be used					internally	Organism part				NULL		0	NULL	NULL	NULL	NULL	NULL	Colloidal Silver is thought to kill an average of 650 different organisms, compared to the 6 of a standard antibiotic.  It is safe for adults, children, animals and pregnant and nursing women. It can be applied topically and used internally and has no reaction with other medications.	topic_mrs
77128	5	355783	11	NULL	NULL	0	NULL	Colloidal Silver	Chemical		is safe for					adults	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Colloidal Silver is thought to kill an average of 650 different organisms, compared to the 6 of a standard antibiotic.  It is safe for adults, children, animals and pregnant and nursing women. It can be applied topically and used internally and has no reaction with other medications.	topic_mrs
77129	6	355783	11	NULL	NULL	0	NULL	Colloidal Silver	Chemical		is safe for					children	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Colloidal Silver is thought to kill an average of 650 different organisms, compared to the 6 of a standard antibiotic.  It is safe for adults, children, animals and pregnant and nursing women. It can be applied topically and used internally and has no reaction with other medications.	topic_mrs
77130	7	355783	11	NULL	NULL	0	NULL	Colloidal Silver 	Chemical		is safe for					animals	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Colloidal Silver is thought to kill an average of 650 different organisms, compared to the 6 of a standard antibiotic.  It is safe for adults, children, animals and pregnant and nursing women. It can be applied topically and used internally and has no reaction with other medications.	topic_mrs
77131	8	355783	11	NULL	NULL	0	NULL	Colloidal Silver	Chemical		is safe for					pregnant women	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Colloidal Silver is thought to kill an average of 650 different organisms, compared to the 6 of a standard antibiotic.  It is safe for adults, children, animals and pregnant and nursing women. It can be applied topically and used internally and has no reaction with other medications.	topic_mrs
77132	9	355783	11	NULL	NULL	0	NULL	Colloidal Silver	Chemical		is safe for					nursing women	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Colloidal Silver is thought to kill an average of 650 different organisms, compared to the 6 of a standard antibiotic.  It is safe for adults, children, animals and pregnant and nursing women. It can be applied topically and used internally and has no reaction with other medications.	topic_mrs
77133	1	355784	11	NULL	NULL	0	NULL	Oleuropein	Chemical		is an ingredient in					Olive Leaf Extract	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Scientific research has shown that the active ingredient in Olive Leaf Extract - Oleuropein, has powerful healing properties that fights the bacteria, viruses, fungi and parasites that cause infection and disease.	topic_mrs
77134	2	355784	11	NULL	NULL	0	NULL	Oleuropein	Chemical		has					healing properties	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Scientific research has shown that the active ingredient in Olive Leaf Extract - Oleuropein, has powerful healing properties that fights the bacteria, viruses, fungi and parasites that cause infection and disease.	topic_mrs
77135	3	355784	11	NULL	NULL	0	NULL	Oleuropein	Chemical		fights with 					bacteria	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Scientific research has shown that the active ingredient in Olive Leaf Extract - Oleuropein, has powerful healing properties that fights the bacteria, viruses, fungi and parasites that cause infection and disease.	topic_mrs
77136	4	355784	11	NULL	NULL	0	NULL	Oleuropein	Chemical		fights with 					viruses	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Scientific research has shown that the active ingredient in Olive Leaf Extract - Oleuropein, has powerful healing properties that fights the bacteria, viruses, fungi and parasites that cause infection and disease.	topic_mrs
77137	5	355784	11	NULL	NULL	0	NULL	Oleuropein	Chemical		fights with 					fungi	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Scientific research has shown that the active ingredient in Olive Leaf Extract - Oleuropein, has powerful healing properties that fights the bacteria, viruses, fungi and parasites that cause infection and disease.	topic_mrs
77138	6	355784	11	NULL	NULL	0	NULL	Oleuropein	Chemical		fights with 					parasites	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Scientific research has shown that the active ingredient in Olive Leaf Extract - Oleuropein, has powerful healing properties that fights the bacteria, viruses, fungi and parasites that cause infection and disease.	topic_mrs
77139	7	355784	11	NULL	NULL	0	NULL	bacteria	Organism		causes					infection	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Scientific research has shown that the active ingredient in Olive Leaf Extract - Oleuropein, has powerful healing properties that fights the bacteria, viruses, fungi and parasites that cause infection and disease.	topic_mrs
77140	8	355784	11	NULL	NULL	0	NULL	Bacteria	Organism		causes					disease	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Scientific research has shown that the active ingredient in Olive Leaf Extract - Oleuropein, has powerful healing properties that fights the bacteria, viruses, fungi and parasites that cause infection and disease.	topic_mrs
77141	9	355784	11	NULL	NULL	0	NULL	viruses	Organism		causes					infection	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Scientific research has shown that the active ingredient in Olive Leaf Extract - Oleuropein, has powerful healing properties that fights the bacteria, viruses, fungi and parasites that cause infection and disease.	topic_mrs
77142	10	355784	11	NULL	NULL	0	NULL	viruses	Organism		causes					disease	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Scientific research has shown that the active ingredient in Olive Leaf Extract - Oleuropein, has powerful healing properties that fights the bacteria, viruses, fungi and parasites that cause infection and disease.	topic_mrs
77143	11	355784	11	NULL	NULL	0	NULL	 fungi	Organism		causes					infection	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Scientific research has shown that the active ingredient in Olive Leaf Extract - Oleuropein, has powerful healing properties that fights the bacteria, viruses, fungi and parasites that cause infection and disease.	topic_mrs
77144	12	355784	11	NULL	NULL	0	NULL	fungi	Organism		causes					disease	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Scientific research has shown that the active ingredient in Olive Leaf Extract - Oleuropein, has powerful healing properties that fights the bacteria, viruses, fungi and parasites that cause infection and disease.	topic_mrs
77145	13	355784	11	NULL	NULL	0	NULL	parasites	Organism		causes					infection	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Scientific research has shown that the active ingredient in Olive Leaf Extract - Oleuropein, has powerful healing properties that fights the bacteria, viruses, fungi and parasites that cause infection and disease.	topic_mrs
77146	14	355784	11	NULL	NULL	0	NULL	parasites	Organism		causes					disease	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Scientific research has shown that the active ingredient in Olive Leaf Extract - Oleuropein, has powerful healing properties that fights the bacteria, viruses, fungi and parasites that cause infection and disease.	topic_mrs
77147	1	355785	11	NULL	NULL	0	NULL	Garlic	Chemical		is a type of 					natural antibiotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Garlic has been scientifically proven to be a powerful natural antibiotic, antiviral and antifungal agent. Garlic has also been shown to kill highly resistant MRSA infections in human clinical studies	topic_mrs
77148	2	355785	11	NULL	NULL	0	NULL	Garlic	Chemical		is a type of 					antiviral agent	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Garlic has been scientifically proven to be a powerful natural antibiotic, antiviral and antifungal agent. Garlic has also been shown to kill highly resistant MRSA infections in human clinical studies	topic_mrs
77149	3	355785	11	NULL	NULL	0	NULL	Garlic	Chemical		is a type of 					 antifungal agent	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Garlic has been scientifically proven to be a powerful natural antibiotic, antiviral and antifungal agent. Garlic has also been shown to kill highly resistant MRSA infections in human clinical studies	topic_mrs
77150	4	355785	11	NULL	NULL	0	NULL	Garlic	Chemical		kills					 MRSA infections	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Garlic has been scientifically proven to be a powerful natural antibiotic, antiviral and antifungal agent. Garlic has also been shown to kill highly resistant MRSA infections in human clinical studies	topic_mrs
77151	1	355786	11	NULL	NULL	NULL	NULL	allicin	Chemical	stabilized 	treats					MRSA infection	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	In 2008, Dr. Ron Cutler and the University of East London  released the results from a human clinical study performed on 52 patients with hospital acquired HA-MRSA. All 52 patients were treated with a form of stabilized allicin and recovered fully from their MRSA infections.	topic_mrs
77152	1	355787	11	NULL	NULL	0	NULL	Manuka honey	Chemical		is a type of 					honey	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Manuka honey is a special medicinal honey that is one of the best natural remedies for Staph and MRSA and has been used for treating infections for over 200 years	topic_mrs
77153	2	355787	11	NULL	NULL	0	NULL	Manuka honey	Chemical		has the property of					medicine	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Manuka honey is a special medicinal honey that is one of the best natural remedies for Staph and MRSA and has been used for treating infections for over 200 years	topic_mrs
77154	3	355787	11	NULL	NULL	0	NULL	Manuka honey	Chemical		treats					staph infections	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Manuka honey is a special medicinal honey that is one of the best natural remedies for Staph and MRSA and has been used for treating infections for over 200 years	topic_mrs
77155	4	355787	11	NULL	NULL	0	NULL	Manuka honey	Chemical		treats					MRSA infection	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Manuka honey is a special medicinal honey that is one of the best natural remedies for Staph and MRSA and has been used for treating infections for over 200 years	topic_mrs
77156	1	355788	11	NULL	NULL	0	NULL	MRSA	Organism		is a type of 					bacterial infections	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Phage Therapy is the therapeutic use of these bacteriophages to treat pathogenic bacterial infections like MRSA. 	topic_mrs
77157	2	355788	11	NULL	NULL	NULL	NULL	Phage Therapy	MedicalProcedure		used in					therapeutic	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Phage Therapy is the therapeutic use of these bacteriophages to treat pathogenic bacterial infections like MRSA. 	topic_mrs
77158	3	355788	11	NULL	NULL	0	NULL	Phage Therapy	MedicalProcedure		treats					bacterial infections	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Phage Therapy is the therapeutic use of these bacteriophages to treat pathogenic bacterial infections like MRSA. 	topic_mrs
77159	1	355789	11	NULL	NULL	0	NULL	Turmeric	Organism		is a type of 					herb	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Turmeric is an herb that contains antibacterial as well as anti-inflammatory properties and has been used to treat boils and other staph infections of the skin, including MRSA, with much success.	topic_mrs
77160	2	355789	11	NULL	NULL	0	NULL	Turmeric	Chemical		has					antibacterial properties	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Turmeric is an herb that contains antibacterial as well as anti-inflammatory properties and has been used to treat boils and other staph infections of the skin, including MRSA, with much success.	topic_mrs
77161	3	355789	11	NULL	NULL	0	NULL	Turmeric	Chemical		has					anti-inflammatory property	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Turmeric is an herb that contains antibacterial as well as anti-inflammatory properties and has been used to treat boils and other staph infections of the skin, including MRSA, with much success.	topic_mrs
77162	4	355789	11	NULL	NULL	0	NULL	Turmeric	Chemical		 treat					boils	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Turmeric is an herb that contains antibacterial as well as anti-inflammatory properties and has been used to treat boils and other staph infections of the skin, including MRSA, with much success.	topic_mrs
77163	5	355789	11	NULL	NULL	0	NULL	Turmeric	Chemical		treats					staph infection	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Turmeric is an herb that contains antibacterial as well as anti-inflammatory properties and has been used to treat boils and other staph infections of the skin, including MRSA, with much success.	topic_mrs
77164	6	355789	11	NULL	NULL	0	NULL	Turmeric	Chemical		treats					MRSA infection	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Turmeric is an herb that contains antibacterial as well as anti-inflammatory properties and has been used to treat boils and other staph infections of the skin, including MRSA, with much success.	topic_mrs
77165	1	355791	11	NULL	NULL	0	NULL	Co-trimoxazole	Chemical		contains					trimethoprim	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Co-trimoxazole is a combination of trimethoprim and sulfamethoxazole, a sulfa drug. It eliminates bacteria that cause various infections, including infections of the urinary tract, lungs (pneumonia), ears, and intestines	topic_mrs
77166	2	355791	11	NULL	NULL	0	NULL	Co-trimoxazole	Chemical		contains					sulfamethoxazole	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Co-trimoxazole is a combination of trimethoprim and sulfamethoxazole, a sulfa drug. It eliminates bacteria that cause various infections, including infections of the urinary tract, lungs (pneumonia), ears, and intestines	topic_mrs
77167	3	355791	11	NULL	NULL	0	NULL	statement 1	Chemical		occurs along with					statement 2	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Co-trimoxazole is a combination of trimethoprim and sulfamethoxazole, a sulfa drug. It eliminates bacteria that cause various infections, including infections of the urinary tract, lungs (pneumonia), ears, and intestines	topic_mrs
77168	4	355791	11	NULL	NULL	0	NULL	sulfamethoxazole	Chemical		is a type of 					sulfa drug	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Co-trimoxazole is a combination of trimethoprim and sulfamethoxazole, a sulfa drug. It eliminates bacteria that cause various infections, including infections of the urinary tract, lungs (pneumonia), ears, and intestines	topic_mrs
77169	5	355791	11	NULL	NULL	0	NULL	bacteria	Organism		infects					urinary tract	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Co-trimoxazole is a combination of trimethoprim and sulfamethoxazole, a sulfa drug. It eliminates bacteria that cause various infections, including infections of the urinary tract, lungs (pneumonia), ears, and intestines	topic_mrs
77170	6	355791	11	NULL	NULL	NULL	NULL	bacteria	Organism		infects					lungs	Organism part				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Co-trimoxazole is a combination of trimethoprim and sulfamethoxazole, a sulfa drug. It eliminates bacteria that cause various infections, including infections of the urinary tract, lungs (pneumonia), ears, and intestines	topic_mrs
77171	7	355791	11	NULL	NULL	0	NULL	pneumonia	MedicalFinding		infects					lungs	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Co-trimoxazole is a combination of trimethoprim and sulfamethoxazole, a sulfa drug. It eliminates bacteria that cause various infections, including infections of the urinary tract, lungs (pneumonia), ears, and intestines	topic_mrs
77172	8	355791	11	NULL	NULL	0	NULL	bacteria	Organism		infects					ears	Organism part				NULL		0	NULL	NULL	NULL	NULL	NULL	Co-trimoxazole is a combination of trimethoprim and sulfamethoxazole, a sulfa drug. It eliminates bacteria that cause various infections, including infections of the urinary tract, lungs (pneumonia), ears, and intestines	topic_mrs
77173	9	355791	11	NULL	NULL	0	NULL	bacteria	Organism		infects					intestines	Organism part				NULL		0	NULL	NULL	NULL	NULL	NULL	Co-trimoxazole is a combination of trimethoprim and sulfamethoxazole, a sulfa drug. It eliminates bacteria that cause various infections, including infections of the urinary tract, lungs (pneumonia), ears, and intestines	topic_mrs
77174	10	355791	11	NULL	NULL	0	NULL	Co-trimoxazole	Chemical		treats					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Co-trimoxazole is a combination of trimethoprim and sulfamethoxazole, a sulfa drug. It eliminates bacteria that cause various infections, including infections of the urinary tract, lungs (pneumonia), ears, and intestines	topic_mrs
77175	11	355791	11	NULL	NULL	0	NULL	Co-trimoxazole	Chemical		treats					statement 6	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Co-trimoxazole is a combination of trimethoprim and sulfamethoxazole, a sulfa drug. It eliminates bacteria that cause various infections, including infections of the urinary tract, lungs (pneumonia), ears, and intestines	topic_mrs
77176	12	355791	11	NULL	NULL	0	NULL	Co-trimoxazole	Chemical		treats					statement 8	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Co-trimoxazole is a combination of trimethoprim and sulfamethoxazole, a sulfa drug. It eliminates bacteria that cause various infections, including infections of the urinary tract, lungs (pneumonia), ears, and intestines	topic_mrs
77177	13	355791	11	NULL	NULL	0	NULL	Co-trimoxazole	Chemical		treats					statement 9	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Co-trimoxazole is a combination of trimethoprim and sulfamethoxazole, a sulfa drug. It eliminates bacteria that cause various infections, including infections of the urinary tract, lungs (pneumonia), ears, and intestines	topic_mrs
77178	1	355792	11	NULL	NULL	0	NULL	Bactrim	Chemical		is a type of 					antibiotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Bactrim (sulfamethoxazole and trimethoprim) is an antibiotic used to treat ear infections, urinary tract and other infections.	topic_mrs
77179	2	355792	11	NULL	NULL	0	NULL	Bactrim	Chemical		contains					sulfamethoxazole	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Bactrim (sulfamethoxazole and trimethoprim) is an antibiotic used to treat ear infections, urinary tract and other infections.	topic_mrs
77180	3	355792	11	NULL	NULL	0	NULL	Bactrim	Chemical		contains					trimethoprim	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Bactrim (sulfamethoxazole and trimethoprim) is an antibiotic used to treat ear infections, urinary tract and other infections.	topic_mrs
77181	4	355792	11	NULL	NULL	0	NULL	statement 2	Chemical		occurs along with					statement 3	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Bactrim (sulfamethoxazole and trimethoprim) is an antibiotic used to treat ear infections, urinary tract and other infections.	topic_mrs
77182	5	355792	11	NULL	NULL	NULL	NULL	Bactrim	Chemical		treats					ear infections	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bactrim (sulfamethoxazole and trimethoprim) is an antibiotic used to treat ear infections, urinary tract and other infections.	topic_mrs
77234	6	355792	11	NULL	NULL	0	NULL	Bactrim	Chemical		treats					urinary tract infections	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Bactrim (sulfamethoxazole and trimethoprim) is an antibiotic used to treat ear infections, urinary tract and other infections.	topic_mrs
77183	1	355793	11	NULL	NULL	0	NULL	Sepsis	MedicalFinding		is a type of 					 illness	Process	 severe			NULL		0	NULL	NULL	NULL	NULL	NULL	Sepsis is a severe illness in which the bloodstream is overwhelmed by bacteria. Sepsis in its most severe form, septic shock, can carry mortality rates well above 50%, even with optimal sepsis treatment.	topic_mrs
77184	2	355793	11	NULL	NULL	0	NULL	sepsis	MedicalFinding	severe	is also known as					 septic shock	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Sepsis is a severe illness in which the bloodstream is overwhelmed by bacteria. Sepsis in its most severe form, septic shock, can carry mortality rates well above 50%, even with optimal sepsis treatment.	topic_mrs
77185	3	355793	11	NULL	NULL	NULL	NULL	 septic shock	MedicalFinding		increases		possibly			mortality	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Sepsis is a severe illness in which the bloodstream is overwhelmed by bacteria. Sepsis in its most severe form, septic shock, can carry mortality rates well above 50%, even with optimal sepsis treatment.	topic_mrs
77186	1	355794	11	NULL	NULL	0	NULL	Antibiotic	Chemical		may cause					diarrhea	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic-associated diarrhea describes frequent, watery bowel movements (diarrhea) that occur in response to medications used to treat bacterial infections (antibiotics)	topic_mrs
77187	2	355794	11	NULL	NULL	0	NULL	diarrhea	MedicalFinding		describes					bowel movements	Process	frequent;;watery			NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic-associated diarrhea describes frequent, watery bowel movements (diarrhea) that occur in response to medications used to treat bacterial infections (antibiotics)	topic_mrs
77188	1	355795	11	NULL	NULL	0	NULL	C. difficile	Organism		is a type of 					bacterium	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	C. difficile is a bacterium that is normally found, along with hundreds of thousands of other bacteria, in the intestines of healthy people.	topic_mrs
77189	2	355795	11	NULL	NULL	0	NULL	C. difficile	Organism		found in					intestines	Organism part	 healthy people			NULL		0	NULL	NULL	NULL	NULL	NULL	C. difficile is a bacterium that is normally found, along with hundreds of thousands of other bacteria, in the intestines of healthy people.	topic_mrs
77190	1	355796	11	NULL	NULL	0	NULL	Clostridium difficile	Organism		is					C. difficile	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	One of the most common causes of antibiotic-associated diarrhea is infection with a bacterium, Clostridium difficile (C. difficile). C. difficile infections are most common in people who are hospitalized, affecting more than 60 hospitalized patients per 100,000 (0.06 percent) in the United States	topic_mrs
77191	2	355796	11	NULL	NULL	0	NULL	Clostridium difficile	Organism		is a type of 					bacterium	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	One of the most common causes of antibiotic-associated diarrhea is infection with a bacterium, Clostridium difficile (C. difficile). C. difficile infections are most common in people who are hospitalized, affecting more than 60 hospitalized patients per 100,000 (0.06 percent) in the United States	topic_mrs
77192	3	355796	11	NULL	NULL	0	NULL	Clostridium difficile	Organism		causes					antibiotic-associated diarrhea	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	One of the most common causes of antibiotic-associated diarrhea is infection with a bacterium, Clostridium difficile (C. difficile). C. difficile infections are most common in people who are hospitalized, affecting more than 60 hospitalized patients per 100,000 (0.06 percent) in the United States	topic_mrs
77193	1	355798	11	NULL	NULL	0	NULL	oral antibiotic	Chemical		treats					C. difficile	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	An oral antibiotic is usually recommended to treat people who are infected with C. difficile.	topic_mrs
78363	1	355800	11	NULL	NULL	0	NULL	antibiotics	Chemical		 related to		possibly			diarrhea	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Some studies have found that probiotics modestly shortened the duration of diarrhea related to antibiotics, but not all patients in these studies had C. difficile	topic_mrs
78364	2	355800	11	NULL	NULL	0	NULL	probiotics	Organism		shortened		modestly			diarrhea	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Some studies have found that probiotics modestly shortened the duration of diarrhea related to antibiotics, but not all patients in these studies had C. difficile	topic_mrs
78365	1	355801	11	NULL	NULL	0	NULL	Hand 	Organism part	washing	prevents					C. difficile	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Hand washing is an effective way to prevent the spread of C. difficile. Hands should be washed after using the bathroom and before eating. 	topic_mrs
78366	1	355802	11	NULL	NULL	0	NULL	Fatigue	MedicalFinding		is also known as					exhaustion	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Fatigue (also called exhaustion, lethargy, languidness, languor, lassitude, and listlessness) is a state of awareness describing a range of afflictions, usually associated with physical and/or mental weakness, though varying from a general state of lethargy to a specific work-induced burning sensation within one's muscles. 	topic_mrs
78367	2	355802	11	NULL	NULL	0	NULL	Fatigue	MedicalFinding		is also known as					 lethargy	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Fatigue (also called exhaustion, lethargy, languidness, languor, lassitude, and listlessness) is a state of awareness describing a range of afflictions, usually associated with physical and/or mental weakness, though varying from a general state of lethargy to a specific work-induced burning sensation within one's muscles. 	topic_mrs
78368	3	355802	11	NULL	NULL	0	NULL	Fatigue	MedicalFinding		is also known as					languidness	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Fatigue (also called exhaustion, lethargy, languidness, languor, lassitude, and listlessness) is a state of awareness describing a range of afflictions, usually associated with physical and/or mental weakness, though varying from a general state of lethargy to a specific work-induced burning sensation within one's muscles. 	topic_mrs
78369	4	355802	11	NULL	NULL	0	NULL	Fatigue	MedicalFinding		is also known as					languor	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Fatigue (also called exhaustion, lethargy, languidness, languor, lassitude, and listlessness) is a state of awareness describing a range of afflictions, usually associated with physical and/or mental weakness, though varying from a general state of lethargy to a specific work-induced burning sensation within one's muscles. 	topic_mrs
78370	5	355802	11	NULL	NULL	0	NULL	Fatigue	MedicalFinding		is also known as					listlessness	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Fatigue (also called exhaustion, lethargy, languidness, languor, lassitude, and listlessness) is a state of awareness describing a range of afflictions, usually associated with physical and/or mental weakness, though varying from a general state of lethargy to a specific work-induced burning sensation within one's muscles. 	topic_mrs
78371	6	355802	11	NULL	NULL	0	NULL	Fatigue 	MedicalFinding		is also known as					lassitude	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Fatigue (also called exhaustion, lethargy, languidness, languor, lassitude, and listlessness) is a state of awareness describing a range of afflictions, usually associated with physical and/or mental weakness, though varying from a general state of lethargy to a specific work-induced burning sensation within one's muscles. 	topic_mrs
78372	7	355802	11	NULL	NULL	0	NULL	Fatigue	MedicalFinding		associated with					weakness	PhysicalPhenomenon	physical;;mental			NULL		0	NULL	NULL	NULL	NULL	NULL	Fatigue (also called exhaustion, lethargy, languidness, languor, lassitude, and listlessness) is a state of awareness describing a range of afflictions, usually associated with physical and/or mental weakness, though varying from a general state of lethargy to a specific work-induced burning sensation within one's muscles. 	topic_mrs
78373	8	355802	11	NULL	NULL	0	NULL	Fatigue	MedicalFinding		 is a state of					awareness	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Fatigue (also called exhaustion, lethargy, languidness, languor, lassitude, and listlessness) is a state of awareness describing a range of afflictions, usually associated with physical and/or mental weakness, though varying from a general state of lethargy to a specific work-induced burning sensation within one's muscles. 	topic_mrs
78374	9	355802	11	NULL	NULL	0	NULL	statement 8	Process		is a range of					afflictions	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Fatigue (also called exhaustion, lethargy, languidness, languor, lassitude, and listlessness) is a state of awareness describing a range of afflictions, usually associated with physical and/or mental weakness, though varying from a general state of lethargy to a specific work-induced burning sensation within one's muscles. 	topic_mrs
78375	10	355802	11	NULL	NULL	0	NULL	work	Process		induced					burning sensation	Process	muscles			NULL		0	NULL	NULL	NULL	NULL	NULL	Fatigue (also called exhaustion, lethargy, languidness, languor, lassitude, and listlessness) is a state of awareness describing a range of afflictions, usually associated with physical and/or mental weakness, though varying from a general state of lethargy to a specific work-induced burning sensation within one's muscles. 	topic_mrs
78376	11	355802	11	NULL	NULL	0	NULL	Fatigue	MedicalFinding		leads to		may			statement 10	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Fatigue (also called exhaustion, lethargy, languidness, languor, lassitude, and listlessness) is a state of awareness describing a range of afflictions, usually associated with physical and/or mental weakness, though varying from a general state of lethargy to a specific work-induced burning sensation within one's muscles. 	topic_mrs
78658	1	355803	11	NULL	NULL	0	NULL	antibiotic	Chemical	short-term	had no effect on		deleterious			aerobic capacity	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We concluded that in healthy individuals, a short-term antibiotic treatment had no deleterious effect on aerobic capacity or on muscle strength and was not associated with subjective side effects	topic_mrs
78659	2	355803	11	NULL	NULL	0	NULL	Antibiotic	Chemical	short-term	had no effect on		deleterious			muscle strength	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We concluded that in healthy individuals, a short-term antibiotic treatment had no deleterious effect on aerobic capacity or on muscle strength and was not associated with subjective side effects	topic_mrs
78660	3	355803	11	NULL	NULL	0	NULL	Antibiotic	Chemical	short-term	was not associated with					side effects	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We concluded that in healthy individuals, a short-term antibiotic treatment had no deleterious effect on aerobic capacity or on muscle strength and was not associated with subjective side effects	topic_mrs
78663	1	355805	11	NULL	NULL	0	NULL	Marijuana	Chemical		is					Cannabis satiVa	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Marijuana (Cannabis satiVa) has long been known to contain antibacterial cannabinoids	topic_mrs
78664	2	355805	11	NULL	NULL	0	NULL	cannabinoids	Chemical		is a type of 					antibacterial	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Marijuana (Cannabis satiVa) has long been known to contain antibacterial cannabinoids	topic_mrs
78665	3	355805	11	NULL	NULL	0	NULL	Marijuana	Chemical		contain					cannabinoids	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Marijuana (Cannabis satiVa) has long been known to contain antibacterial cannabinoids	topic_mrs
76311	1	355807	5	11	NULL	NULL	NULL	DNMT3A gene	GP	mutation of	is associated with					AML	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	According to research published in the November 11 issue of the New England Journal of Medicine, researchers sequenced the genome of a patient who died of AML, then compared that genome to those of 281 other patients, and found that over 20% of them shared this mutation, at a gene known as DNMT3A, 	topic_ll
78666	1	355807	5	11	NULL	0	NULL	DNMT3A	GP	mutation of	published in					New England Journal of Medicine	Journal				NULL		0	NULL	NULL	NULL	NULL	NULL	According to research published in the November 11 issue of the New England Journal of Medicine, researchers sequenced the genome of a patient who died of AML, then compared that genome to those of 281 other patients, and found that over 20% of them shared this mutation, at a gene known as DNMT3A, 	topic_ll
78667	1	355808	5	11	NULL	0	NULL	glands	Organism part		produces					saliva	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Biopsying the glands that produce saliva to test for germinal center-like formation when someone is diagnosed with primary Sjögren’s Syndrome can predict later development of non-Hodgkin’s lymphoma, according to research presented this week at the American College of Rheumatology Annual Scientific Meeting in Atlanta.	topic_ll
76312	1	355809	5	NULL	NULL	0	NULL	NHL	MedicalFinding		is					non-Hodgkin lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	"Some patients with non-Hodgkin lymphoma (NHL) - a cancer of B cells - harbor a particular mutation in the gene encoding the receptor for B cell activating factor (BAFF), 	topic_ll
76313	2	355809	5	NULL	NULL	0	NULL	BAFF	GP		is					B cell activating factor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	"Some patients with non-Hodgkin lymphoma (NHL) - a cancer of B cells - harbor a particular mutation in the gene encoding the receptor for B cell activating factor (BAFF), 	topic_ll
76314	3	355809	5	NULL	NULL	0	NULL	NHL	MedicalFinding		is a type of					cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	"Some patients with non-Hodgkin lymphoma (NHL) - a cancer of B cells - harbor a particular mutation in the gene encoding the receptor for B cell activating factor (BAFF), 	topic_ll
76315	4	355809	5	11	NULL	NULL	NULL	NHL	MedicalFinding		affects					B cells	Cell				NULL		NULL	NULL	NULL	NULL	NULL	NULL	"Some patients with non-Hodgkin lymphoma (NHL) - a cancer of B cells - harbor a particular mutation in the gene encoding the receptor for B cell activating factor (BAFF), 	topic_ll
76316	5	355809	5	11	NULL	NULL	NULL	BAFF receptor	GP	mutation of	leads to					NHL	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	"Some patients with non-Hodgkin lymphoma (NHL) - a cancer of B cells - harbor a particular mutation in the gene encoding the receptor for B cell activating factor (BAFF), 	topic_ll
78668	1	355809	5	11	NULL	0	NULL	non-Hodgkin lymphoma	MedicalFinding		is					NHL	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	"Some patients with non-Hodgkin lymphoma (NHL) - a cancer of B cells - harbor a particular mutation in the gene encoding the receptor for B cell activating factor (BAFF), 	topic_ll
78669	1	355809	5	11	NULL	NULL	NULL	non-Hodgkin lymphoma	MedicalFinding		is a type of 					cancer	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	"Some patients with non-Hodgkin lymphoma (NHL) - a cancer of B cells - harbor a particular mutation in the gene encoding the receptor for B cell activating factor (BAFF), 	topic_ll
78670	1	355809	5	11	NULL	0	NULL	 B cell activating factor	GP		is					BAFF	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	"Some patients with non-Hodgkin lymphoma (NHL) - a cancer of B cells - harbor a particular mutation in the gene encoding the receptor for B cell activating factor (BAFF), 	topic_ll
76317	1	355810	5	11	NULL	NULL	NULL	sun tanning	Process		is linked to		may be			lymphomas	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Over the years, several peer-reviewed medical studies have attempted to establish a link between sun tanning and lymphomas, with the verdict closely split down the middle.	topic_ll
76318	1	355812	5	NULL	NULL	0	NULL	DHA	Chemical		is a type of					cosmetic ingredient	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The FDA approves DHA as a cosmetic ingredient, and it has no known direct connection to causing lymphomas or any other type of disease.	topic_ll
76319	2	355812	5	NULL	NULL	0	NULL	FDA	GroupOfPeople		approves					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The FDA approves DHA as a cosmetic ingredient, and it has no known direct connection to causing lymphomas or any other type of disease.	topic_ll
76320	3	355812	5	NULL	NULL	0	NULL	DHA	Chemical		does not cause					lymphomas	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The FDA approves DHA as a cosmetic ingredient, and it has no known direct connection to causing lymphomas or any other type of disease.	topic_ll
76321	1	355814	5	NULL	NULL	0	NULL	DHA	Chemical		is					Dihydroxyacetone	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	they usually contain a substance called DHA (Dihydroxyacetone), which stains the outer layer of dead skin cells a darker color.	topic_ll
76322	2	355814	5	NULL	NULL	0	NULL	skin	OrganismPart	outer layer of;;dead	is stained					darker color	AbstractConcept				NULL		0	NULL	NULL	NULL	NULL	NULL	they usually contain a substance called DHA (Dihydroxyacetone), which stains the outer layer of dead skin cells a darker color.	topic_ll
76323	3	355814	5	NULL	NULL	0	NULL	DHA	Chemical		is required for					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	they usually contain a substance called DHA (Dihydroxyacetone), which stains the outer layer of dead skin cells a darker color.	topic_ll
76324	1	355815	5	NULL	NULL	0	NULL	HHV6	GP	presence of	indicator of		predicting			cellular immunosuppression	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of HHV6 can be considered as a predicting indicator of cellular immunosuppression preceding the onset of CMV infection which may result in a severe outcome among pediatric lymphoma patients.	topic_ll
76325	2	355815	5	NULL	NULL	0	NULL	cellular immunosuppression	MedicalFinding		precedes					CMV infection	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of HHV6 can be considered as a predicting indicator of cellular immunosuppression preceding the onset of CMV infection which may result in a severe outcome among pediatric lymphoma patients.	topic_ll
76326	3	355815	5	NULL	NULL	0	NULL	statement 2	Process		results in		may			pediatric lymphoma patients	GroupOfPeople	severe outcome of			NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of HHV6 can be considered as a predicting indicator of cellular immunosuppression preceding the onset of CMV infection which may result in a severe outcome among pediatric lymphoma patients.	topic_ll
76585	1	355817	5	NULL	NULL	0	NULL	cancers	MedicalFinding	secondary	is not uncommon for					Hodgkin's patients	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Since secondary cancers are not uncommon for Hodgkin's patients anywhere from 5-25 years down the road due to exposure to chemo and radiation, this study suggests that many patients are being overtreated at the current guidelines and that the lower chemo and radiation levels should be considered. 	topic_ll
76586	2	355817	5	NULL	NULL	0	NULL	chemo	MedicalProcedure	exposure to	causes					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Since secondary cancers are not uncommon for Hodgkin's patients anywhere from 5-25 years down the road due to exposure to chemo and radiation, this study suggests that many patients are being overtreated at the current guidelines and that the lower chemo and radiation levels should be considered. 	topic_ll
76587	3	355817	5	NULL	NULL	0	NULL	radiation	PhysicalPhenomenon	exposure to	causes					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Since secondary cancers are not uncommon for Hodgkin's patients anywhere from 5-25 years down the road due to exposure to chemo and radiation, this study suggests that many patients are being overtreated at the current guidelines and that the lower chemo and radiation levels should be considered. 	topic_ll
76588	1	355818	5	NULL	NULL	0	NULL	FDG	Chemical	high rates of	exists in					T-cell lymphomas	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	They determined that high rates of FDG positivity did indeed exist in T-cell lymphomas and "given the propensity for disease involvement outside the normal scan range of diagnostic CT, we recommend that patients with T-cell lymphoma be scanned from vertex to feet by use of PET/CT.	topic_ll
76589	2	355818	5	NULL	NULL	0	NULL	T-cell lymphoma patients	GroupOfPeople		scanned from					vertex	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	They determined that high rates of FDG positivity did indeed exist in T-cell lymphomas and "given the propensity for disease involvement outside the normal scan range of diagnostic CT, we recommend that patients with T-cell lymphoma be scanned from vertex to feet by use of PET/CT.	topic_ll
76590	3	355818	5	NULL	NULL	0	NULL	T-cell lymphoma patients	GroupOfPeople		scanned to					feet	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	They determined that high rates of FDG positivity did indeed exist in T-cell lymphomas and "given the propensity for disease involvement outside the normal scan range of diagnostic CT, we recommend that patients with T-cell lymphoma be scanned from vertex to feet by use of PET/CT.	topic_ll
76591	4	355818	5	NULL	NULL	0	NULL	statement 2	Process		occurs along with					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	They determined that high rates of FDG positivity did indeed exist in T-cell lymphomas and "given the propensity for disease involvement outside the normal scan range of diagnostic CT, we recommend that patients with T-cell lymphoma be scanned from vertex to feet by use of PET/CT.	topic_ll
76592	5	355818	5	NULL	NULL	0	NULL	PET/CT	MedicalProcedure		is used for					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	They determined that high rates of FDG positivity did indeed exist in T-cell lymphomas and "given the propensity for disease involvement outside the normal scan range of diagnostic CT, we recommend that patients with T-cell lymphoma be scanned from vertex to feet by use of PET/CT.	topic_ll
76593	6	355818	5	NULL	NULL	0	NULL	PET/CT	MedicalProcedure		is used for					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	They determined that high rates of FDG positivity did indeed exist in T-cell lymphomas and "given the propensity for disease involvement outside the normal scan range of diagnostic CT, we recommend that patients with T-cell lymphoma be scanned from vertex to feet by use of PET/CT.	topic_ll
76594	1	355819	5	NULL	NULL	0	NULL	PET-CT	MedicalProcedure	extended	is recommended for					T-cell lymphomas	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Extended PET-CT recommended for T-cell lymphomas 	topic_ll
76673	1	355820	7	NULL	NULL	0	NULL	FDG	Chemical		used during					 PET-CT scan	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	FDG (fluorodeoxyglucose) is the radiopharmaceutical agent used during a PET-CT scan 	topic_ll
76674	2	355820	7	NULL	NULL	0	NULL	FDG	Chemical		is a type of					radiopharmaceutical agent	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	FDG (fluorodeoxyglucose) is the radiopharmaceutical agent used during a PET-CT scan 	topic_ll
76675	3	355820	7	NULL	NULL	0	NULL	FDG	Chemical		is					fluorodeoxyglucose	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	FDG (fluorodeoxyglucose) is the radiopharmaceutical agent used during a PET-CT scan 	topic_ll
76676	1	355821	7	NULL	NULL	0	NULL	social rhythm therapy	MedicalProcedure		added to					interpersonal psychotherapy	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of social rhythm therapy to interpersonal psychotherapy leads to create a new psychotherapy adaptated to bipolar disorders: InterPersonal and Social Rhythm Therapy (IPSRT).	topic_bd
76677	2	355821	7	NULL	NULL	NULL	NULL	statement 1	Process		leads to					IPSRT	MedicalProcedure				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Addition of social rhythm therapy to interpersonal psychotherapy leads to create a new psychotherapy adaptated to bipolar disorders: InterPersonal and Social Rhythm Therapy (IPSRT).	topic_bd
76678	3	355821	7	NULL	NULL	0	NULL	statement 2	Process		adaptated to					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of social rhythm therapy to interpersonal psychotherapy leads to create a new psychotherapy adaptated to bipolar disorders: InterPersonal and Social Rhythm Therapy (IPSRT).	topic_bd
76679	4	355821	7	NULL	NULL	0	NULL	IPSRT	MedicalProcedure		is a type of					new psychotherapy	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of social rhythm therapy to interpersonal psychotherapy leads to create a new psychotherapy adaptated to bipolar disorders: InterPersonal and Social Rhythm Therapy (IPSRT).	topic_bd
76680	5	355821	7	NULL	NULL	0	NULL	IPSRT	MedicalProcedure		is					InterPersonal and Social Rhythm Therapy	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of social rhythm therapy to interpersonal psychotherapy leads to create a new psychotherapy adaptated to bipolar disorders: InterPersonal and Social Rhythm Therapy (IPSRT).	topic_bd
76688	1	355822	7	NULL	NULL	0	NULL	rTMS	MedicalProcedure		used in the 					mood episodes	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	Thus, treating mood episodes and fighting against resistant and residual symptoms or chronicity of the disorders constitute major clinical issues and economic challenges. They have generated great interest in finding new non-pharmacological approaches such as repetitive transcranial magnetic stimulation (rTMS).	topic_bd
76689	2	355822	7	NULL	NULL	0	NULL	rTMS	MedicalProcedure		is					repetitive transcranial magnetic stimulation	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Thus, treating mood episodes and fighting against resistant and residual symptoms or chronicity of the disorders constitute major clinical issues and economic challenges. They have generated great interest in finding new non-pharmacological approaches such as repetitive transcranial magnetic stimulation (rTMS).	topic_bd
76690	3	355822	7	NULL	NULL	0	NULL	rTMS	MedicalProcedure		is a type of					non-pharmacological approach	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Thus, treating mood episodes and fighting against resistant and residual symptoms or chronicity of the disorders constitute major clinical issues and economic challenges. They have generated great interest in finding new non-pharmacological approaches such as repetitive transcranial magnetic stimulation (rTMS).	topic_bd
76681	1	355824	7	NULL	NULL	0	NULL	dorsolateral prefrontal cortex	OrganismPart	left side of	have effect in					mood control	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Given the hypothesis that the right and left sides of the dorsolateral prefrontal cortex have opposing effects in mood control, high-frequency rTMS activates the left side and low-frequency to inhibit the right side in the treatment of depression.	topic_bd
76682	2	355824	7	NULL	NULL	NULL	NULL	dorsolateral prefrontal cortex	OrganismPart	right side of	have effect in					mood control	MentalProcess				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Given the hypothesis that the right and left sides of the dorsolateral prefrontal cortex have opposing effects in mood control, high-frequency rTMS activates the left side and low-frequency to inhibit the right side in the treatment of depression.	topic_bd
76683	3	355824	7	NULL	NULL	0	NULL	statement 1	Process		opposing effect to					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Given the hypothesis that the right and left sides of the dorsolateral prefrontal cortex have opposing effects in mood control, high-frequency rTMS activates the left side and low-frequency to inhibit the right side in the treatment of depression.	topic_bd
76684	4	355824	7	NULL	NULL	NULL	NULL	rTMS	MedicalProcedure	high-frequency	activates 					dorsolateral prefrontal cortex	OrganismPart	left side of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Given the hypothesis that the right and left sides of the dorsolateral prefrontal cortex have opposing effects in mood control, high-frequency rTMS activates the left side and low-frequency to inhibit the right side in the treatment of depression.	topic_bd
76685	5	355824	7	NULL	NULL	0	NULL	rTMS	MedicalProcedure	low-frequency	inhibit					dorsolateral prefrontal cortex	OrganismPart	right side of			NULL		0	NULL	NULL	NULL	NULL	NULL	Given the hypothesis that the right and left sides of the dorsolateral prefrontal cortex have opposing effects in mood control, high-frequency rTMS activates the left side and low-frequency to inhibit the right side in the treatment of depression.	topic_bd
76686	6	355824	7	NULL	NULL	0	NULL	statement 4	Process		in the treatment of					depression	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Given the hypothesis that the right and left sides of the dorsolateral prefrontal cortex have opposing effects in mood control, high-frequency rTMS activates the left side and low-frequency to inhibit the right side in the treatment of depression.	topic_bd
76687	7	355824	7	NULL	NULL	0	NULL	statement 5	Process		in the treatment of					depression	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Given the hypothesis that the right and left sides of the dorsolateral prefrontal cortex have opposing effects in mood control, high-frequency rTMS activates the left side and low-frequency to inhibit the right side in the treatment of depression.	topic_bd
76862	1	355825	7	NULL	NULL	0	NULL	rTMS 	MedicalProcedure		effective in the					bipolar depression	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	Overall, rTMS seems to be effective in the treatment of bipolar depression but further trials with larger cohorts should determine optimal parameters of stimulation.	topic_bd
76863	1	355826	7	NULL	NULL	0	NULL	vVBM	MedicalProcedure	optimized	shows					bipolar I disorder	MedicalFinding	smaller volumes in the left inferior parietal lobule			NULL		0	NULL	NULL	NULL	NULL	NULL	There was no difference in whole-brain gray matter volume between the two groups. Optimized vVBM showed that subjects with bipolar I disorder had smaller volumes in the left inferior parietal lobule, right superior temporal gyrus, right middle frontal gyrus and left caudate	topic_bd
76864	2	355826	7	NULL	NULL	0	NULL	 vVBM	MedicalProcedure	optimized	shows					bipolar I disorder	MedicalFinding	smaller volumes in right superior temporal gyrus			NULL		0	NULL	NULL	NULL	NULL	NULL	There was no difference in whole-brain gray matter volume between the two groups. Optimized vVBM showed that subjects with bipolar I disorder had smaller volumes in the left inferior parietal lobule, right superior temporal gyrus, right middle frontal gyrus and left caudate	topic_bd
76865	3	355826	7	NULL	NULL	NULL	NULL	vVBM	MedicalProcedure	optimized	shows					bipolar I disorder	MedicalFinding	small volumes in right  middle frontal gyrus			NULL		NULL	NULL	NULL	NULL	NULL	NULL	There was no difference in whole-brain gray matter volume between the two groups. Optimized vVBM showed that subjects with bipolar I disorder had smaller volumes in the left inferior parietal lobule, right superior temporal gyrus, right middle frontal gyrus and left caudate	topic_bd
76866	4	355826	7	NULL	NULL	0	NULL	vVBM	MedicalProcedure	optimized	shows					bipolar I disorder	MedicalFinding	smaller volumes in left caudate			NULL		0	NULL	NULL	NULL	NULL	NULL	There was no difference in whole-brain gray matter volume between the two groups. Optimized vVBM showed that subjects with bipolar I disorder had smaller volumes in the left inferior parietal lobule, right superior temporal gyrus, right middle frontal gyrus and left caudate	topic_bd
76867	1	355827	7	NULL	NULL	0	NULL	gray matter defects	OrganismPart		seen in					bipolar I disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest widespread gray matter defects in bipolar I disorder, which may play an important role in onset of the illness.	topic_bd
76868	2	355827	7	NULL	NULL	0	NULL	statement 1	Process		important role in					illness	MedicalFinding	onset of			NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest widespread gray matter defects in bipolar I disorder, which may play an important role in onset of the illness.	topic_bd
76869	1	355830	7	NULL	NULL	0	NULL	lintuzumab	Chemical		failed to 					survival	Process	demonstrate overall			NULL		0	NULL	NULL	NULL	NULL	NULL	A Phase IIb study of the monoclonal antibody lintuzumab, also known as SGN33, failed to demonstrate an improvement in overall survival compared to current chemotherapy	topic_ll
76870	2	355830	7	NULL	NULL	0	NULL	lintuzumab	Chemical		is known as					SGN33	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	A Phase IIb study of the monoclonal antibody lintuzumab, also known as SGN33, failed to demonstrate an improvement in overall survival compared to current chemotherapy	topic_ll
76871	3	355830	7	NULL	NULL	0	NULL	lintuzumab	Chemical		is a type of					monoclonal antibody	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	A Phase IIb study of the monoclonal antibody lintuzumab, also known as SGN33, failed to demonstrate an improvement in overall survival compared to current chemotherapy	topic_ll
76872	1	355831	7	NULL	NULL	0	NULL	children	GroupOfPeople	older father	risk of					NHLs	MedicalFinding	developing			NULL		0	NULL	NULL	NULL	NULL	NULL	Now a new and possibly unique study out of City of Hope Hospital in southern California suggests kids of born of older fathers are at an increased risk of developing NHLs.	topic_ll
76873	1	355832	7	NULL	NULL	0	NULL	Shark cartilage extract	GP		does not produce					anti-cancer effects	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Shark cartilage extract produces no anti-cancer effects in latest study	topic_ll
76874	1	355833	7	NULL	NULL	0	NULL	brentuximab vedotin	Chemical		is a type of					anti-cancer drug	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Seattle Genetics is reporting positive preliminary results from a phase II trial of its promising anti-cancer drug brentuximab vedotin (SGN-35) against patients with anaplastic large cell lymphoma, (ALCL)	topic_ll
76875	2	355833	7	NULL	NULL	0	NULL	brentuximab vedotin	Chemical		against					ALCL	MedicalFinding	patients with			NULL		0	NULL	NULL	NULL	NULL	NULL	Seattle Genetics is reporting positive preliminary results from a phase II trial of its promising anti-cancer drug brentuximab vedotin (SGN-35) against patients with anaplastic large cell lymphoma, (ALCL)	topic_ll
76876	3	355833	7	NULL	NULL	0	NULL	ALCL	MedicalFinding		is					anaplastic large cell lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Seattle Genetics is reporting positive preliminary results from a phase II trial of its promising anti-cancer drug brentuximab vedotin (SGN-35) against patients with anaplastic large cell lymphoma, (ALCL)	topic_ll
76877	4	355833	7	NULL	NULL	0	NULL	 brentuximab vedotin 	Chemical		is known as					SGN-35	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Seattle Genetics is reporting positive preliminary results from a phase II trial of its promising anti-cancer drug brentuximab vedotin (SGN-35) against patients with anaplastic large cell lymphoma, (ALCL)	topic_ll
76878	1	355834	7	NULL	NULL	0	NULL	brentuximab vedotin	Chemical		is used for					relapsed Hodgkin's lymphoma	MedicalFinding	patients with			NULL		0	NULL	NULL	NULL	NULL	NULL	Seattle Genetics has announced top-line results from a phase II trial of its antibody-drug conjugate (ADC) brentuximab vedotin (SGN-35) for patients with relapsed or refractory Hodgkin's lymphoma	topic_ll
76879	2	355834	7	NULL	NULL	NULL	NULL	brentuximab vedotin	Chemical		is used for					refractory Hodgkin's lymphoma	MedicalFinding	patients with			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Seattle Genetics has announced top-line results from a phase II trial of its antibody-drug conjugate (ADC) brentuximab vedotin (SGN-35) for patients with relapsed or refractory Hodgkin's lymphoma	topic_ll
76880	3	355834	7	NULL	NULL	0	NULL	brentuximab vedotin 	Chemical		is a type of					ADC	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Seattle Genetics has announced top-line results from a phase II trial of its antibody-drug conjugate (ADC) brentuximab vedotin (SGN-35) for patients with relapsed or refractory Hodgkin's lymphoma	topic_ll
76881	4	355834	7	NULL	NULL	0	NULL	ADC	Chemical		is					antibody-drug conjugate	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Seattle Genetics has announced top-line results from a phase II trial of its antibody-drug conjugate (ADC) brentuximab vedotin (SGN-35) for patients with relapsed or refractory Hodgkin's lymphoma	topic_ll
76882	5	355834	7	NULL	NULL	0	NULL	brentuximab vedotin	Chemical		is known as					SGN-35	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Seattle Genetics has announced top-line results from a phase II trial of its antibody-drug conjugate (ADC) brentuximab vedotin (SGN-35) for patients with relapsed or refractory Hodgkin's lymphoma	topic_ll
76883	1	355835	7	NULL	NULL	0	NULL	Personalized Lymphoma Vaccine	Chemical		prevent					follicular lymphoma patients	MedicalFinding	recurrence among			NULL		0	NULL	NULL	NULL	NULL	NULL	Personalized Lymphoma Vaccine Increases Survival by Two Years A personalized vaccine is a powerful therapy to prevent recurrence among certain follicular lymphoma patients, according to the latest results of ongoing research led by the University of Pennsylvania School of Medicine.	topic_ll
76884	2	355835	7	NULL	NULL	0	NULL	Personalized Lymphoma Vaccine	MedicalFinding		increase					follicular lymphoma patients	MedicalFinding	survival of			NULL		0	NULL	NULL	NULL	NULL	NULL	Personalized Lymphoma Vaccine Increases Survival by Two Years A personalized vaccine is a powerful therapy to prevent recurrence among certain follicular lymphoma patients, according to the latest results of ongoing research led by the University of Pennsylvania School of Medicine.	topic_ll
76885	1	355837	7	NULL	NULL	0	NULL	Omapro	Chemical		used for					CML	MedicalFinding	patients with			NULL		0	NULL	NULL	NULL	NULL	NULL	a diagnostic test to identify patients with the T3151 genetic mutation prior to giving approval to ChemGenex Pharmaceuticals' Omapro (omacetaxine) as a treatment for patients with chronic myeloid leukemia (CML) who did not respond to initial treatment with Gleevec (imatinib).	topic_ll
76886	2	355837	7	NULL	NULL	0	NULL	Omapro	Chemical		is					omacetaxine	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	a diagnostic test to identify patients with the T3151 genetic mutation prior to giving approval to ChemGenex Pharmaceuticals' Omapro (omacetaxine) as a treatment for patients with chronic myeloid leukemia (CML) who did not respond to initial treatment with Gleevec (imatinib).	topic_ll
76887	3	355837	7	NULL	NULL	NULL	NULL	CML patients	MedicalFinding		did not respond to					Gleevec	Chemical	initial treatment with			NULL		NULL	NULL	NULL	NULL	NULL	NULL	a diagnostic test to identify patients with the T3151 genetic mutation prior to giving approval to ChemGenex Pharmaceuticals' Omapro (omacetaxine) as a treatment for patients with chronic myeloid leukemia (CML) who did not respond to initial treatment with Gleevec (imatinib).	topic_ll
76888	4	355837	7	NULL	NULL	0	NULL	Omapro	Chemical		is used in					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	a diagnostic test to identify patients with the T3151 genetic mutation prior to giving approval to ChemGenex Pharmaceuticals' Omapro (omacetaxine) as a treatment for patients with chronic myeloid leukemia (CML) who did not respond to initial treatment with Gleevec (imatinib).	topic_ll
76889	5	355837	7	NULL	NULL	0	NULL	CML	MedicalFinding		is					chronic myeloid leukemia 	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	a diagnostic test to identify patients with the T3151 genetic mutation prior to giving approval to ChemGenex Pharmaceuticals' Omapro (omacetaxine) as a treatment for patients with chronic myeloid leukemia (CML) who did not respond to initial treatment with Gleevec (imatinib).	topic_ll
76896	6	355837	7	NULL	NULL	0	NULL	Gleevec	Chemical		is					imatinib	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	a diagnostic test to identify patients with the T3151 genetic mutation prior to giving approval to ChemGenex Pharmaceuticals' Omapro (omacetaxine) as a treatment for patients with chronic myeloid leukemia (CML) who did not respond to initial treatment with Gleevec (imatinib).	topic_ll
76890	1	355838	7	NULL	NULL	0	NULL	GVAX Leukemia Vaccine	Chemical		reduces		severly			cancer cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	GVAX Leukemia Vaccine either severely reduces or completely eliminates cancer cells remaining in some patients with chronic myeloid leukemia (CML) who have been on Gleevec for a year or longer.	topic_ll
76891	2	355838	7	NULL	NULL	0	NULL	GVAX Leukemia Vaccine	Chemical		eliminates		completely			cancer cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	GVAX Leukemia Vaccine either severely reduces or completely eliminates cancer cells remaining in some patients with chronic myeloid leukemia (CML) who have been on Gleevec for a year or longer.	topic_ll
76892	3	355838	7	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	GVAX Leukemia Vaccine either severely reduces or completely eliminates cancer cells remaining in some patients with chronic myeloid leukemia (CML) who have been on Gleevec for a year or longer.	topic_ll
76893	5	355838	7	NULL	NULL	NULL	NULL	statement 3	Process		in patients with					statement 4	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	GVAX Leukemia Vaccine either severely reduces or completely eliminates cancer cells remaining in some patients with chronic myeloid leukemia (CML) who have been on Gleevec for a year or longer.	topic_ll
76894	4	355838	7	NULL	NULL	NULL	NULL	Gleevec	Chemical		used in the					CML	MedicalFinding	treatment of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	GVAX Leukemia Vaccine either severely reduces or completely eliminates cancer cells remaining in some patients with chronic myeloid leukemia (CML) who have been on Gleevec for a year or longer.	topic_ll
76895	6	355838	7	NULL	NULL	0	NULL	CML	MedicalFinding		is					chronic myeloid leukemia 	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	GVAX Leukemia Vaccine either severely reduces or completely eliminates cancer cells remaining in some patients with chronic myeloid leukemia (CML) who have been on Gleevec for a year or longer.	topic_ll
76897	1	355840	7	NULL	NULL	0	NULL	tumors	Cell		have					CD68-positive macrophages	Cell	high number of			NULL		0	NULL	NULL	NULL	NULL	NULL	The minority of patients who relapse and sometimes die if they don't receive more aggressive therapy appear to have something in their tumors the others don't: a high number of white cells called CD68-positive macrophages (scavenger cells). It appears that the more of these cells in the tumor, the shorter the 10-year survival rate, the more aggressive the secondary treatment required. 	topic_ll
76898	2	355840	7	NULL	NULL	0	NULL	statement 1	Process		leads to					 survival rate	Process	shorter			NULL		0	NULL	NULL	NULL	NULL	NULL	The minority of patients who relapse and sometimes die if they don't receive more aggressive therapy appear to have something in their tumors the others don't: a high number of white cells called CD68-positive macrophages (scavenger cells). It appears that the more of these cells in the tumor, the shorter the 10-year survival rate, the more aggressive the secondary treatment required. 	topic_ll
76899	3	355840	7	NULL	NULL	0	NULL	statement 1	Process		requires					secondary treatment 	MedicalProcedure	aggressive			NULL		0	NULL	NULL	NULL	NULL	NULL	The minority of patients who relapse and sometimes die if they don't receive more aggressive therapy appear to have something in their tumors the others don't: a high number of white cells called CD68-positive macrophages (scavenger cells). It appears that the more of these cells in the tumor, the shorter the 10-year survival rate, the more aggressive the secondary treatment required. 	topic_ll
76900	4	355840	7	NULL	NULL	0	NULL	CD68-positive macrophages	Cell		is a type of					white cells 	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	The minority of patients who relapse and sometimes die if they don't receive more aggressive therapy appear to have something in their tumors the others don't: a high number of white cells called CD68-positive macrophages (scavenger cells). It appears that the more of these cells in the tumor, the shorter the 10-year survival rate, the more aggressive the secondary treatment required. 	topic_ll
76901	5	355840	7	NULL	NULL	0	NULL	CD68-positive macrophages	Cell		is a type of					scavenger cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	The minority of patients who relapse and sometimes die if they don't receive more aggressive therapy appear to have something in their tumors the others don't: a high number of white cells called CD68-positive macrophages (scavenger cells). It appears that the more of these cells in the tumor, the shorter the 10-year survival rate, the more aggressive the secondary treatment required. 	topic_ll
76902	1	355841	7	NULL	NULL	0	NULL	natural sunlight	Chemical		produce					vitamin D	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Research conducted in this area reveals the fact that exposure to natural sunlight produces vitamin D that helps fight against symptoms of non-Hodgkin's lymphoma.	topic_ll
76903	2	355841	7	NULL	NULL	0	NULL	statement 1	Process		helps in					non-Hodgkin's lymphoma	MedicalFinding	fight against symptoms of			NULL		0	NULL	NULL	NULL	NULL	NULL	Research conducted in this area reveals the fact that exposure to natural sunlight produces vitamin D that helps fight against symptoms of non-Hodgkin's lymphoma.	topic_ll
76904	1	355842	7	NULL	NULL	NULL	NULL	Non-Hodgkins lymphoma	MedicalFinding	treatment of	include		may			Reishi mushroom	Organism	use of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Non-Hodgkin’s lymphoma and Hodgkin’s lymphoma treatments may include the use of Reishi mushroom, green tea, olive leaf, milk thistle, and standardized extract.	topic_ll
76905	2	355842	7	NULL	NULL	NULL	NULL	Non-Hodgkins lymphoma	MedicalFinding	treatment of	include		may			green tea	Organism	use of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Non-Hodgkin’s lymphoma and Hodgkin’s lymphoma treatments may include the use of Reishi mushroom, green tea, olive leaf, milk thistle, and standardized extract.	topic_ll
76906	3	355842	7	NULL	NULL	NULL	NULL	Non-Hodgkins lymphoma	MedicalFinding	treatment of	include		may			milk thistle	Organism	use of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Non-Hodgkin’s lymphoma and Hodgkin’s lymphoma treatments may include the use of Reishi mushroom, green tea, olive leaf, milk thistle, and standardized extract.	topic_ll
76907	5	355842	7	NULL	NULL	NULL	NULL	Hodgkins lymphoma	MedicalFinding	treatment of	include		may			Reishi mushroom	Organism	use of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Non-Hodgkin’s lymphoma and Hodgkin’s lymphoma treatments may include the use of Reishi mushroom, green tea, olive leaf, milk thistle, and standardized extract.	topic_ll
76908	4	355842	7	NULL	NULL	NULL	NULL	Non-Hodgkins lymphoma 	MedicalFinding	treatment of	include		may			olive leaf	OrganismPart	use of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Non-Hodgkin’s lymphoma and Hodgkin’s lymphoma treatments may include the use of Reishi mushroom, green tea, olive leaf, milk thistle, and standardized extract.	topic_ll
76909	6	355842	7	NULL	NULL	0	NULL	Hodgkins lymphoma	MedicalFinding	treatment of	include		may			green tea	Organism	use of			NULL		0	NULL	NULL	NULL	NULL	NULL	Non-Hodgkin’s lymphoma and Hodgkin’s lymphoma treatments may include the use of Reishi mushroom, green tea, olive leaf, milk thistle, and standardized extract.	topic_ll
76910	7	355842	7	NULL	NULL	0	NULL	Hodgkins lymphoma	MedicalFinding	treatment of	include		may			olive leaf	OrganismPart	use of			NULL		0	NULL	NULL	NULL	NULL	NULL	Non-Hodgkin’s lymphoma and Hodgkin’s lymphoma treatments may include the use of Reishi mushroom, green tea, olive leaf, milk thistle, and standardized extract.	topic_ll
76911	8	355842	7	NULL	NULL	0	NULL	Hodgkins lymphoma	MedicalFinding		include		may			milk thistle	Organism	use of			NULL		0	NULL	NULL	NULL	NULL	NULL	Non-Hodgkin’s lymphoma and Hodgkin’s lymphoma treatments may include the use of Reishi mushroom, green tea, olive leaf, milk thistle, and standardized extract.	topic_ll
76912	1	355846	7	NULL	NULL	0	NULL	SHIP	GP		suppress					B cell lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Protein ID'ed May Help with Lymphoma Therapies SHIP and PTEN act cooperatively to suppress B cell lymphoma.	topic_ll
76913	2	355846	7	NULL	NULL	NULL	NULL	PTEN	GP		suppress					B cell lymphoma	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Protein ID'ed May Help with Lymphoma Therapies SHIP and PTEN act cooperatively to suppress B cell lymphoma.	topic_ll
76914	3	355846	7	NULL	NULL	0	NULL	statement 1	Process		in cooperation with					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Protein ID'ed May Help with Lymphoma Therapies SHIP and PTEN act cooperatively to suppress B cell lymphoma.	topic_ll
77048	1	355847	7	NULL	NULL	0	NULL	SHIP	GP		act in cooperation with					PTEN	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammatory Diseases Program at Sanford-Burnham Medical Research Institute (Sanford-Burnham), explores the roles of two enzymes, called SHIP and PTEN, in B cell growth and proliferation.Protein ID'ed May Help with Lymphoma Therapies SHIP and PTEN act cooperatively to suppress B cell lymphoma. 	topic_ll
77049	2	355847	7	NULL	NULL	0	NULL	statement 1	Process		suppress					B cell lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammatory Diseases Program at Sanford-Burnham Medical Research Institute (Sanford-Burnham), explores the roles of two enzymes, called SHIP and PTEN, in B cell growth and proliferation.Protein ID'ed May Help with Lymphoma Therapies SHIP and PTEN act cooperatively to suppress B cell lymphoma. 	topic_ll
77050	3	355847	7	NULL	NULL	0	NULL	SHIP	GP		is a type of					enzyme	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammatory Diseases Program at Sanford-Burnham Medical Research Institute (Sanford-Burnham), explores the roles of two enzymes, called SHIP and PTEN, in B cell growth and proliferation.Protein ID'ed May Help with Lymphoma Therapies SHIP and PTEN act cooperatively to suppress B cell lymphoma. 	topic_ll
77051	4	355847	7	NULL	NULL	0	NULL	PTEN	GP		is a type of					enzyme	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammatory Diseases Program at Sanford-Burnham Medical Research Institute (Sanford-Burnham), explores the roles of two enzymes, called SHIP and PTEN, in B cell growth and proliferation.Protein ID'ed May Help with Lymphoma Therapies SHIP and PTEN act cooperatively to suppress B cell lymphoma. 	topic_ll
77052	1	355850	7	NULL	NULL	0	NULL	 primary central nervous system lymphoma	MedicalFinding	prognosis of	poor					therapy	MedicalProcedure	regardless of			NULL		0	NULL	NULL	NULL	NULL	NULL	Noting that the prognosis for most patients with primary central nervous system lymphoma is poor regardless of therapy and that only a minority of patients achieve a complete response to current chemotherapy regimens, Mayo Clinic researchers carried out a randomized phase II clinical trial in which high-dose cytarabine was added to high-dose methotrexate . 	topic_ll
77053	1	355853	7	NULL	NULL	0	NULL	ENMD-2076	Chemical		used to					AML	MedicalFinding	treat			NULL		0	NULL	NULL	NULL	NULL	NULL	The US FDA has granted orphan-drug status to EntreMed's ENMD-2076, the company's lead cancer drug candidate designed to treat acute myeloid leukemia (AML). 	topic_ll
77054	2	355853	7	NULL	NULL	0	NULL	AML	MedicalFinding		is					acute myeloid leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The US FDA has granted orphan-drug status to EntreMed's ENMD-2076, the company's lead cancer drug candidate designed to treat acute myeloid leukemia (AML). 	topic_ll
77090	1	355855	7	NULL	NULL	0	NULL	British garden rhubarb 	Organism	baking of	raise					polyphenols	Chemical	levels of			NULL		0	NULL	NULL	NULL	NULL	NULL	Findings published in the journal Food Chemistry suggest that baking a specific variety of British garden rhubarb grown in South Yorkshire for just 20 minutes raises the level of anti-cancerous chemicals known as polyphenols found in the plant.	topic_ll
77091	2	355855	7	NULL	NULL	0	NULL	polyphenols	Chemical		is a type of					anti-cancerous chemicals	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Findings published in the journal Food Chemistry suggest that baking a specific variety of British garden rhubarb grown in South Yorkshire for just 20 minutes raises the level of anti-cancerous chemicals known as polyphenols found in the plant.	topic_ll
77092	1	355857	7	NULL	NULL	0	NULL	Polyphenols	Chemical		kills					cancer cells	Cell	active			NULL		0	NULL	NULL	NULL	NULL	NULL	Polyphenols have been shown in the past to be active cancer cell killers and researchers from the Biomedical Research Centre of Sheffield Hallam University believe there may be some potential benefit to applying these findings to a less toxic treatment for certain leukemias, even those proven to be resistant to current treatment	topic_ll
77093	1	355860	7	NULL	NULL	0	NULL	yellow/orange fruits	Food		associated with					NHL	MedicalFinding	lower risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	Greater intake of total fruits and vegetables, yellow/orange and cruciferous vegetables, broccoli and apple juice/cider are associated with a lower NHL risk, although this was only observed for follicular lymphoma, not in DLBCL.	topic_ll
77094	2	355860	7	NULL	NULL	NULL	NULL	cruciferous vegetables	Food		associated with					NHL	MedicalFinding	lower risk of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Greater intake of total fruits and vegetables, yellow/orange and cruciferous vegetables, broccoli and apple juice/cider are associated with a lower NHL risk, although this was only observed for follicular lymphoma, not in DLBCL.	topic_ll
77095	3	355860	7	NULL	NULL	0	NULL	broccoli 	Food		associated with					NHL	MedicalFinding	lower risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	Greater intake of total fruits and vegetables, yellow/orange and cruciferous vegetables, broccoli and apple juice/cider are associated with a lower NHL risk, although this was only observed for follicular lymphoma, not in DLBCL.	topic_ll
77096	4	355860	7	NULL	NULL	0	NULL	apple juice/cider	Food		associated with					NHL	MedicalFinding	lower risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	Greater intake of total fruits and vegetables, yellow/orange and cruciferous vegetables, broccoli and apple juice/cider are associated with a lower NHL risk, although this was only observed for follicular lymphoma, not in DLBCL.	topic_ll
77097	5	355860	7	NULL	NULL	0	NULL	statement 1	Process		observed in					follicular lymphoma 	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Greater intake of total fruits and vegetables, yellow/orange and cruciferous vegetables, broccoli and apple juice/cider are associated with a lower NHL risk, although this was only observed for follicular lymphoma, not in DLBCL.	topic_ll
77098	6	355860	7	NULL	NULL	NULL	NULL	statement 2	Process		observed in					follicular lymphoma 	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Greater intake of total fruits and vegetables, yellow/orange and cruciferous vegetables, broccoli and apple juice/cider are associated with a lower NHL risk, although this was only observed for follicular lymphoma, not in DLBCL.	topic_ll
77099	7	355860	7	NULL	NULL	0	NULL	statement 3	Process		observed in					follicular lymphoma 	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Greater intake of total fruits and vegetables, yellow/orange and cruciferous vegetables, broccoli and apple juice/cider are associated with a lower NHL risk, although this was only observed for follicular lymphoma, not in DLBCL.	topic_ll
77100	8	355860	7	NULL	NULL	0	NULL	statement 4	Process		observed in					follicular lymphoma 	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Greater intake of total fruits and vegetables, yellow/orange and cruciferous vegetables, broccoli and apple juice/cider are associated with a lower NHL risk, although this was only observed for follicular lymphoma, not in DLBCL.	topic_ll
77101	9	355860	7	NULL	NULL	0	NULL	statement 1	Process		not observed in					DLBCL	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Greater intake of total fruits and vegetables, yellow/orange and cruciferous vegetables, broccoli and apple juice/cider are associated with a lower NHL risk, although this was only observed for follicular lymphoma, not in DLBCL.	topic_ll
77102	10	355860	7	NULL	NULL	0	NULL	statement 2	Process		not observed in					DLBCL	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Greater intake of total fruits and vegetables, yellow/orange and cruciferous vegetables, broccoli and apple juice/cider are associated with a lower NHL risk, although this was only observed for follicular lymphoma, not in DLBCL.	topic_ll
77103	11	355860	7	NULL	NULL	0	NULL	statement 3	Process		not observed in					DLBCL	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Greater intake of total fruits and vegetables, yellow/orange and cruciferous vegetables, broccoli and apple juice/cider are associated with a lower NHL risk, although this was only observed for follicular lymphoma, not in DLBCL.	topic_ll
77104	12	355860	7	NULL	NULL	0	NULL	statement 4	Process		not observed in					DLBCL	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Greater intake of total fruits and vegetables, yellow/orange and cruciferous vegetables, broccoli and apple juice/cider are associated with a lower NHL risk, although this was only observed for follicular lymphoma, not in DLBCL.	topic_ll
77105	1	355864	7	NULL	NULL	0	NULL	B cells	Cell	desensitization of	occur by					antigen receptors	GP	inactivating			NULL		0	NULL	NULL	NULL	NULL	NULL	National Jewish Health has been issued a US patent claiming a method to desensitize B cells by inactivating antigen receptors on their surfaces. The method, discovered by John Cambier, PhD, Chairman of the Integrated Department of Immunology at National Jewish Health, holds promise for treatment of B-cell mediated diseases, such as lymphoma and leukemia	topic_ll
77106	2	355864	7	NULL	NULL	0	NULL	antigen receptors 	GP		present on					B cells	Cell	surface of			NULL		0	NULL	NULL	NULL	NULL	NULL	National Jewish Health has been issued a US patent claiming a method to desensitize B cells by inactivating antigen receptors on their surfaces. The method, discovered by John Cambier, PhD, Chairman of the Integrated Department of Immunology at National Jewish Health, holds promise for treatment of B-cell mediated diseases, such as lymphoma and leukemia	topic_ll
77107	3	355864	7	NULL	NULL	0	NULL	statement 1	Process		used in the					lymphoma	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	National Jewish Health has been issued a US patent claiming a method to desensitize B cells by inactivating antigen receptors on their surfaces. The method, discovered by John Cambier, PhD, Chairman of the Integrated Department of Immunology at National Jewish Health, holds promise for treatment of B-cell mediated diseases, such as lymphoma and leukemia	topic_ll
77108	4	355864	7	NULL	NULL	0	NULL	statement 1	Process		used in the					leukemia	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	National Jewish Health has been issued a US patent claiming a method to desensitize B cells by inactivating antigen receptors on their surfaces. The method, discovered by John Cambier, PhD, Chairman of the Integrated Department of Immunology at National Jewish Health, holds promise for treatment of B-cell mediated diseases, such as lymphoma and leukemia	topic_ll
77109	5	355864	7	NULL	NULL	0	NULL	lymphoma	MedicalFinding		is a type of					B-cell mediated diseases	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	National Jewish Health has been issued a US patent claiming a method to desensitize B cells by inactivating antigen receptors on their surfaces. The method, discovered by John Cambier, PhD, Chairman of the Integrated Department of Immunology at National Jewish Health, holds promise for treatment of B-cell mediated diseases, such as lymphoma and leukemia	topic_ll
77110	6	355864	7	NULL	NULL	0	NULL	leukemia	MedicalFinding		is a type of					B-cell mediated diseases	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	National Jewish Health has been issued a US patent claiming a method to desensitize B cells by inactivating antigen receptors on their surfaces. The method, discovered by John Cambier, PhD, Chairman of the Integrated Department of Immunology at National Jewish Health, holds promise for treatment of B-cell mediated diseases, such as lymphoma and leukemia	topic_ll
77111	1	355865	7	NULL	NULL	NULL	NULL	MALT1	GP		boost 					 DLBCL	MedicalFinding	effectiveness of treatment against			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Working independently of one another, two groups of researchers have uncovered a possible strategy involving a protease enzyme known as MALT1 to boost the effectiveness of treatment against diffuse large B-cell lymphoma (DLBCL), 	topic_ll
77112	2	355865	7	NULL	NULL	0	NULL	DLBCL	MedicalFinding		is					diffuse large B-cell lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Working independently of one another, two groups of researchers have uncovered a possible strategy involving a protease enzyme known as MALT1 to boost the effectiveness of treatment against diffuse large B-cell lymphoma (DLBCL), 	topic_ll
77113	3	355865	7	NULL	NULL	0	NULL	MALT1	GP		is a type of					protease enzyme	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Working independently of one another, two groups of researchers have uncovered a possible strategy involving a protease enzyme known as MALT1 to boost the effectiveness of treatment against diffuse large B-cell lymphoma (DLBCL), 	topic_ll
77114	1	355867	7	NULL	NULL	0	NULL	romidepsin	Chemical		used in the					CTCL	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	Earlier this month, the US FDA approved the antibiotic histone deacetylase inhibitor romidepsin (marketed as Istodax injection) for treating patients with cutaneous T-cell lymphoma (CTCL) who have undergone at least one prior systemic therapy. 	topic_ll
77115	2	355867	7	NULL	NULL	0	NULL	CTCL	MedicalFinding		is					cutaneous T-cell lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Earlier this month, the US FDA approved the antibiotic histone deacetylase inhibitor romidepsin (marketed as Istodax injection) for treating patients with cutaneous T-cell lymphoma (CTCL) who have undergone at least one prior systemic therapy. 	topic_ll
77116	3	355867	7	NULL	NULL	0	NULL	romidepsin	Chemical		is a type of					histone deacetylase inhibitor	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Earlier this month, the US FDA approved the antibiotic histone deacetylase inhibitor romidepsin (marketed as Istodax injection) for treating patients with cutaneous T-cell lymphoma (CTCL) who have undergone at least one prior systemic therapy. 	topic_ll
77117	4	355867	7	NULL	NULL	0	NULL	romidepsin	Chemical		is a type of					antibiotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Earlier this month, the US FDA approved the antibiotic histone deacetylase inhibitor romidepsin (marketed as Istodax injection) for treating patients with cutaneous T-cell lymphoma (CTCL) who have undergone at least one prior systemic therapy. 	topic_ll
77118	1	355869	7	NULL	NULL	0	NULL	Bendamustine	Chemical		used to treat					iNHL	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Results from a study published in the journal Cancer suggest that patients with indolent B-cell non-Hodgkin’s lymphoma (iNHL) are responding well to Bendamustine, a chemo drug generally used to treat chronic lymphocytocic leukemia and some NHLs. 	topic_ll
77119	2	355869	7	NULL	NULL	0	NULL	Bendamustine	Chemical		used to treat					chronic lymphocytocic leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Results from a study published in the journal Cancer suggest that patients with indolent B-cell non-Hodgkin’s lymphoma (iNHL) are responding well to Bendamustine, a chemo drug generally used to treat chronic lymphocytocic leukemia and some NHLs. 	topic_ll
77120	3	355869	7	NULL	NULL	0	NULL	Bendamustine	Chemical		used to treat					NHL	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Results from a study published in the journal Cancer suggest that patients with indolent B-cell non-Hodgkin’s lymphoma (iNHL) are responding well to Bendamustine, a chemo drug generally used to treat chronic lymphocytocic leukemia and some NHLs. 	topic_ll
77121	4	355869	7	NULL	NULL	NULL	NULL	iNHL	MedicalFinding		is 					indolent B-cell non-Hodgkins lymphoma	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Results from a study published in the journal Cancer suggest that patients with indolent B-cell non-Hodgkin’s lymphoma (iNHL) are responding well to Bendamustine, a chemo drug generally used to treat chronic lymphocytocic leukemia and some NHLs. 	topic_ll
77122	5	355869	7	NULL	NULL	0	NULL	Bendamustine	Chemical		is a type of					chemodrug	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Results from a study published in the journal Cancer suggest that patients with indolent B-cell non-Hodgkin’s lymphoma (iNHL) are responding well to Bendamustine, a chemo drug generally used to treat chronic lymphocytocic leukemia and some NHLs. 	topic_ll
77123	1	355871	7	NULL	NULL	0	NULL	X-rays 	MedicalProcedure	exposure to	associated with					ALL	MedicalFinding	children with			NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically, the researchers found that children with acute lymphoid leukemia (ALL) had almost twice the chance of having been exposed to three or more X-rays compared with children who did not have leukemia.	topic_ll
77124	2	355871	7	NULL	NULL	0	NULL	ALL	MedicalFinding		is					acute lymphoid leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically, the researchers found that children with acute lymphoid leukemia (ALL) had almost twice the chance of having been exposed to three or more X-rays compared with children who did not have leukemia.	topic_ll
77194	1	355872	7	NULL	NULL	NULL	NULL	X-rays	MedicalProcedure		increase					ALL	MedicalFinding	risk for			NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study found an increased risk from X-rays for ALL, but not for AML or T-cell leukemia, and there was no association with age at first exposure.	topic_ll
77195	2	355872	7	NULL	NULL	0	NULL	X-rays	MedicalProcedure		does not increase					AML	MedicalFinding	risk for			NULL		0	NULL	NULL	NULL	NULL	NULL	The study found an increased risk from X-rays for ALL, but not for AML or T-cell leukemia, and there was no association with age at first exposure.	topic_ll
77196	3	355872	7	NULL	NULL	NULL	NULL	X-rays	MedicalProcedure		does not increase					T-cell leukemia	MedicalFinding	risk for			NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study found an increased risk from X-rays for ALL, but not for AML or T-cell leukemia, and there was no association with age at first exposure.	topic_ll
77197	1	355873	7	NULL	NULL	0	NULL	Fmn2 gene	GP	excessive synthesis of	associated with					B-cell lymphocytic leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Charfi first compared the transcriptome (the set of active genes in a cell) of leukemic and healthy mice. From this analysis, she was able to isolate groups of genes with abnormal activity in the leukemic mice. This led to the discovery that excessive synthesis of the Fmn2 gene and protein is associated with B-cell lymphocytic leukemia.	topic_ll
77198	2	355873	7	NULL	NULL	0	NULL	Fmn2 protein	GP	excessive synthesis of	associated with					B-cell lymphocytic leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Charfi first compared the transcriptome (the set of active genes in a cell) of leukemic and healthy mice. From this analysis, she was able to isolate groups of genes with abnormal activity in the leukemic mice. This led to the discovery that excessive synthesis of the Fmn2 gene and protein is associated with B-cell lymphocytic leukemia.	topic_ll
77199	1	355875	7	NULL	NULL	0	NULL	IL-7 	GP		trigger					B cells	Cell	maturation of			NULL		0	NULL	NULL	NULL	NULL	NULL	Upon closer evaluation, the research team found that Miz-1 has a very particular function: it is required for IL-7 to effectively trigger the maturation of B cells in the bone marrow. 	topic_ll
77200	2	355875	7	NULL	NULL	0	NULL	statement 1	Process		occur in					bone marrow	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Upon closer evaluation, the research team found that Miz-1 has a very particular function: it is required for IL-7 to effectively trigger the maturation of B cells in the bone marrow. 	topic_ll
77201	3	355875	7	NULL	NULL	0	NULL	Miz-1	GP		required for					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Upon closer evaluation, the research team found that Miz-1 has a very particular function: it is required for IL-7 to effectively trigger the maturation of B cells in the bone marrow. 	topic_ll
77202	1	355877	7	NULL	NULL	0	NULL	brain tumors 	MedicalFinding	low-grade	have					IDH gene	GP	mutated version of			NULL		0	NULL	NULL	NULL	NULL	NULL	About 75 percent of people with low-grade brain tumors and 20 percent of people with acute myeloid leukemia have a mutated version of a gene known as IDH.	topic_ll
77203	2	355877	7	NULL	NULL	0	NULL	acute myeloid leukemia	MedicalFinding		have					IDH gene	GP	mutated version of			NULL		0	NULL	NULL	NULL	NULL	NULL	About 75 percent of people with low-grade brain tumors and 20 percent of people with acute myeloid leukemia have a mutated version of a gene known as IDH.	topic_ll
77204	1	355878	7	NULL	NULL	NULL	NULL	IDH	GP	cells with mutation of	produce					α-KG	GP				NULL		NULL	NULL	NULL	NULL	NULL	NULL	The researchers discovered that cells with the IDH mutation produce less α-KG and more 2-HG than normal cells. 2-HG then outcompetes α-KG, disabling a whole family of enzymes that depend on α-KG to do their jobs in the cell. Normal cell functions break down, contributing to the development of cancer.	topic_ll
77205	2	355878	7	NULL	NULL	NULL	NULL	IDH	GP	cells with mutation of	produce					 2-HG	GP				NULL		NULL	NULL	NULL	NULL	NULL	NULL	The researchers discovered that cells with the IDH mutation produce less α-KG and more 2-HG than normal cells. 2-HG then outcompetes α-KG, disabling a whole family of enzymes that depend on α-KG to do their jobs in the cell. Normal cell functions break down, contributing to the development of cancer.	topic_ll
77206	3	355878	7	NULL	NULL	NULL	NULL	normal cells	Cell		produce					α-KG 	GP				NULL		NULL	NULL	NULL	NULL	NULL	NULL	The researchers discovered that cells with the IDH mutation produce less α-KG and more 2-HG than normal cells. 2-HG then outcompetes α-KG, disabling a whole family of enzymes that depend on α-KG to do their jobs in the cell. Normal cell functions break down, contributing to the development of cancer.	topic_ll
77207	4	355878	7	NULL	NULL	0	NULL	normal cells	Cell		produce					 2-HG 	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The researchers discovered that cells with the IDH mutation produce less α-KG and more 2-HG than normal cells. 2-HG then outcompetes α-KG, disabling a whole family of enzymes that depend on α-KG to do their jobs in the cell. Normal cell functions break down, contributing to the development of cancer.	topic_ll
77208	5	355878	7	NULL	NULL	0	NULL	statement 1	Process		is less compared to					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The researchers discovered that cells with the IDH mutation produce less α-KG and more 2-HG than normal cells. 2-HG then outcompetes α-KG, disabling a whole family of enzymes that depend on α-KG to do their jobs in the cell. Normal cell functions break down, contributing to the development of cancer.	topic_ll
77209	6	355878	7	NULL	NULL	0	NULL	statement 2	Process		is more compared to					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The researchers discovered that cells with the IDH mutation produce less α-KG and more 2-HG than normal cells. 2-HG then outcompetes α-KG, disabling a whole family of enzymes that depend on α-KG to do their jobs in the cell. Normal cell functions break down, contributing to the development of cancer.	topic_ll
77210	7	355878	7	NULL	NULL	0	NULL	Normal cell	Cell		functions					breakdown	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The researchers discovered that cells with the IDH mutation produce less α-KG and more 2-HG than normal cells. 2-HG then outcompetes α-KG, disabling a whole family of enzymes that depend on α-KG to do their jobs in the cell. Normal cell functions break down, contributing to the development of cancer.	topic_ll
77211	8	355878	7	NULL	NULL	0	NULL	statement 7	Process		contributes to					cancer	MedicalFinding	development of			NULL		0	NULL	NULL	NULL	NULL	NULL	The researchers discovered that cells with the IDH mutation produce less α-KG and more 2-HG than normal cells. 2-HG then outcompetes α-KG, disabling a whole family of enzymes that depend on α-KG to do their jobs in the cell. Normal cell functions break down, contributing to the development of cancer.	topic_ll
77212	1	355879	7	NULL	NULL	0	NULL	RG7112	Chemical		used to treat					refractory acute leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with relapsed or refractory acute or chronic leukemia were given RG7112 orally each day for 10 days, followed by 18 days of rest. Forty-seven patients, including 27 with acute myeloid leukemia (AML), have been treated to date.	topic_ll
77213	2	355879	7	NULL	NULL	0	NULL	RG7112	Chemical		used to treat					refractory chronic leukemia 	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with relapsed or refractory acute or chronic leukemia were given RG7112 orally each day for 10 days, followed by 18 days of rest. Forty-seven patients, including 27 with acute myeloid leukemia (AML), have been treated to date.	topic_ll
77214	3	355879	7	NULL	NULL	0	NULL	AML	MedicalFinding		is					acute myeloid leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with relapsed or refractory acute or chronic leukemia were given RG7112 orally each day for 10 days, followed by 18 days of rest. Forty-seven patients, including 27 with acute myeloid leukemia (AML), have been treated to date.	topic_ll
77215	4	355879	7	NULL	NULL	0	NULL	RG7112 	Chemical		used to treat					relapsed acute leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with relapsed or refractory acute or chronic leukemia were given RG7112 orally each day for 10 days, followed by 18 days of rest. Forty-seven patients, including 27 with acute myeloid leukemia (AML), have been treated to date.	topic_ll
77216	5	355879	7	NULL	NULL	0	NULL	RG7112	Chemical		used to treat					relapsed chronic leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with relapsed or refractory acute or chronic leukemia were given RG7112 orally each day for 10 days, followed by 18 days of rest. Forty-seven patients, including 27 with acute myeloid leukemia (AML), have been treated to date.	topic_ll
77217	1	355880	7	NULL	NULL	0	NULL	RG7112	Chemical		used to treat					relapsed acute leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with relapsed or refractory acute or chronic leukemia were given RG7112 orally each day for 10 days, followed by 18 days of rest. Forty-seven patients, including 27 with acute myeloid leukemia (AML), have been treated to date. The drug used in this study, RG7112, a novel small molecule being developed by Roche, is a member of the Nutlin family.	topic_ll
77218	2	355880	7	NULL	NULL	0	NULL	RG7112	Chemical		used to treat					relapsed chronic leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with relapsed or refractory acute or chronic leukemia were given RG7112 orally each day for 10 days, followed by 18 days of rest. Forty-seven patients, including 27 with acute myeloid leukemia (AML), have been treated to date. The drug used in this study, RG7112, a novel small molecule being developed by Roche, is a member of the Nutlin family.	topic_ll
77219	3	355880	7	NULL	NULL	0	NULL	RG7112	Chemical		used to treat					refractory acute leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with relapsed or refractory acute or chronic leukemia were given RG7112 orally each day for 10 days, followed by 18 days of rest. Forty-seven patients, including 27 with acute myeloid leukemia (AML), have been treated to date. The drug used in this study, RG7112, a novel small molecule being developed by Roche, is a member of the Nutlin family.	topic_ll
77220	4	355880	7	NULL	NULL	0	NULL	RG7112	Chemical		used to treat					refractory chronic leukemia 	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with relapsed or refractory acute or chronic leukemia were given RG7112 orally each day for 10 days, followed by 18 days of rest. Forty-seven patients, including 27 with acute myeloid leukemia (AML), have been treated to date. The drug used in this study, RG7112, a novel small molecule being developed by Roche, is a member of the Nutlin family.	topic_ll
77221	5	355880	7	NULL	NULL	0	NULL	AML	MedicalFinding		is					acute myeloid leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with relapsed or refractory acute or chronic leukemia were given RG7112 orally each day for 10 days, followed by 18 days of rest. Forty-seven patients, including 27 with acute myeloid leukemia (AML), have been treated to date. The drug used in this study, RG7112, a novel small molecule being developed by Roche, is a member of the Nutlin family.	topic_ll
77222	6	355880	7	NULL	NULL	0	NULL	RG7112	Chemical		is a member of					Nutlin family	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with relapsed or refractory acute or chronic leukemia were given RG7112 orally each day for 10 days, followed by 18 days of rest. Forty-seven patients, including 27 with acute myeloid leukemia (AML), have been treated to date. The drug used in this study, RG7112, a novel small molecule being developed by Roche, is a member of the Nutlin family.	topic_ll
77223	1	355881	7	NULL	NULL	0	NULL	TP53 gene 	GP	mutations of	rare in					blood	OrganismPart	cancers of			NULL		0	NULL	NULL	NULL	NULL	NULL	While mutations of the TP53 gene are rare in cancers of the blood, the p53 protein may be degraded by other factors, including high levels of MDM2, which binds to p53 and orchestrates its degradation.	topic_ll
77224	2	355881	7	NULL	NULL	0	NULL	MDM2	GP	high levels of	degrade		may 			p53 protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	While mutations of the TP53 gene are rare in cancers of the blood, the p53 protein may be degraded by other factors, including high levels of MDM2, which binds to p53 and orchestrates its degradation.	topic_ll
77225	3	355881	7	NULL	NULL	0	NULL	MDM2	GP		bind					p53	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	While mutations of the TP53 gene are rare in cancers of the blood, the p53 protein may be degraded by other factors, including high levels of MDM2, which binds to p53 and orchestrates its degradation.	topic_ll
77226	4	355881	7	NULL	NULL	0	NULL	statement 3	Process		orchestrates					p53	GP	degradation of			NULL		0	NULL	NULL	NULL	NULL	NULL	While mutations of the TP53 gene are rare in cancers of the blood, the p53 protein may be degraded by other factors, including high levels of MDM2, which binds to p53 and orchestrates its degradation.	topic_ll
77227	1	355882	7	NULL	NULL	0	NULL	Small Molecule	Chemical		disarm		may			Cancer-Fighting P53	GP	 Enemy of			NULL		0	NULL	NULL	NULL	NULL	NULL	Small Molecule May Disarm Enemy of Cancer-Fighting P53	topic_ll
77228	1	355883	7	NULL	NULL	0	NULL	Nutlins	Chemical		effective in					leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In preclinical studies, small-molecule MDM2 antagonists called Nutlins were found to be effective in solid tumors, leukemia and lymphoma.	topic_ll
77229	2	355883	7	NULL	NULL	0	NULL	Nutlins	Chemical		effective in					lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In preclinical studies, small-molecule MDM2 antagonists called Nutlins were found to be effective in solid tumors, leukemia and lymphoma.	topic_ll
77230	3	355883	7	NULL	NULL	0	NULL	Nutlins	Chemical		is a type of					MDM2 antagonists	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	In preclinical studies, small-molecule MDM2 antagonists called Nutlins were found to be effective in solid tumors, leukemia and lymphoma.	topic_ll
77231	4	355883	7	NULL	NULL	0	NULL	Nutlins	Chemical		is a type of					small molecule	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	In preclinical studies, small-molecule MDM2 antagonists called Nutlins were found to be effective in solid tumors, leukemia and lymphoma.	topic_ll
77232	5	355883	7	NULL	NULL	0	NULL	leukemia	MedicalFinding		is a type of					solid tumor	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In preclinical studies, small-molecule MDM2 antagonists called Nutlins were found to be effective in solid tumors, leukemia and lymphoma.	topic_ll
77233	6	355883	7	NULL	NULL	0	NULL	lymphoma	MedicalFinding		is a type of					solid tumor	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In preclinical studies, small-molecule MDM2 antagonists called Nutlins were found to be effective in solid tumors, leukemia and lymphoma.	topic_ll
77255	1	355884	7	NULL	NULL	0	NULL	RG7112	Chemical		is a type of					novel small molecule	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The drug used in this study, RG7112, a novel small molecule being developed by Roche, is a member of the Nutlin family.	topic_ll
77256	2	355884	7	NULL	NULL	0	NULL	RG7112	Chemical		is a member of					Nutlin family	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The drug used in this study, RG7112, a novel small molecule being developed by Roche, is a member of the Nutlin family.	topic_ll
77257	1	355885	7	NULL	NULL	NULL	NULL	lymph node	OrganismPart	Reduction in	seen in					CLL	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Reductions in lymph node and spleen size, as well as in circulating leukemia cells, were seen in chronic lymphocytic leukemia (CLL) and small lymphocytic lymphoma (SLL).	topic_ll
77258	2	355885	7	NULL	NULL	NULL	NULL	spleen	OrganismPart	reduction in size of	seen in					CLL	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Reductions in lymph node and spleen size, as well as in circulating leukemia cells, were seen in chronic lymphocytic leukemia (CLL) and small lymphocytic lymphoma (SLL).	topic_ll
77259	3	355885	7	NULL	NULL	0	NULL	circulating leukemia cells	Cell	reduction in	seen in					CLL	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Reductions in lymph node and spleen size, as well as in circulating leukemia cells, were seen in chronic lymphocytic leukemia (CLL) and small lymphocytic lymphoma (SLL).	topic_ll
77260	4	355885	7	NULL	NULL	0	NULL	lymph node	OrganismPart	reduction in	seen in					SLL	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Reductions in lymph node and spleen size, as well as in circulating leukemia cells, were seen in chronic lymphocytic leukemia (CLL) and small lymphocytic lymphoma (SLL).	topic_ll
77261	5	355885	7	NULL	NULL	0	NULL	spleen	OrganismPart	reduction in size of	seen in					SLL	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Reductions in lymph node and spleen size, as well as in circulating leukemia cells, were seen in chronic lymphocytic leukemia (CLL) and small lymphocytic lymphoma (SLL).	topic_ll
77262	6	355885	7	NULL	NULL	0	NULL	circulating leukemia cells	Cell	reduction in	seen in					SLL	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Reductions in lymph node and spleen size, as well as in circulating leukemia cells, were seen in chronic lymphocytic leukemia (CLL) and small lymphocytic lymphoma (SLL).	topic_ll
77263	7	355885	7	NULL	NULL	0	NULL	CLL	MedicalFinding		is					chronic lymphocytic leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Reductions in lymph node and spleen size, as well as in circulating leukemia cells, were seen in chronic lymphocytic leukemia (CLL) and small lymphocytic lymphoma (SLL).	topic_ll
77264	8	355885	7	NULL	NULL	0	NULL	SLL	MedicalFinding		is					small lymphocytic lymphoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Reductions in lymph node and spleen size, as well as in circulating leukemia cells, were seen in chronic lymphocytic leukemia (CLL) and small lymphocytic lymphoma (SLL).	topic_ll
77265	1	355886	7	NULL	NULL	0	NULL	AAK	GP		essential for					cell division	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	AAK is essential for cell division (mitotic progression) and is amplified or overexpressed in AML and other blood cancers.	topic_ll
77266	2	355886	7	NULL	NULL	0	NULL	cell division 	Process		is					mitotic progression	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	AAK is essential for cell division (mitotic progression) and is amplified or overexpressed in AML and other blood cancers.	topic_ll
77267	3	355886	7	NULL	NULL	0	NULL	AAK	GP		overexpressed in					AML	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	AAK is essential for cell division (mitotic progression) and is amplified or overexpressed in AML and other blood cancers.	topic_ll
77268	4	355886	7	NULL	NULL	0	NULL	AAK	GP		overexpressed in					blood cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	AAK is essential for cell division (mitotic progression) and is amplified or overexpressed in AML and other blood cancers.	topic_ll
77269	5	355886	7	NULL	NULL	0	NULL	AAK	GP		amplified in					AML	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	AAK is essential for cell division (mitotic progression) and is amplified or overexpressed in AML and other blood cancers.	topic_ll
77270	6	355886	7	NULL	NULL	0	NULL	AAK	GP		amplified in					blood cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	AAK is essential for cell division (mitotic progression) and is amplified or overexpressed in AML and other blood cancers.	topic_ll
77271	7	355886	7	NULL	NULL	0	NULL	statement 3	Process		is an alternative to					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	AAK is essential for cell division (mitotic progression) and is amplified or overexpressed in AML and other blood cancers.	topic_ll
77272	8	355886	7	NULL	NULL	0	NULL	statement 4	Process		is an alternative to					statement 6	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	AAK is essential for cell division (mitotic progression) and is amplified or overexpressed in AML and other blood cancers.	topic_ll
77273	1	355887	7	NULL	NULL	NULL	NULL	MLN8237 	Chemical		inhibitor of		potent;;selective			AAK	GP				NULL		NULL	NULL	NULL	NULL	NULL	NULL	An investigational drug, MLN8237 is an orally available, potent, and selective AAK inhibitor. It has shown preclinical activity against leukemia, lymphoma,	topic_ll
77274	2	355887	7	NULL	NULL	0	NULL	statement 1	Process		shows					leukemia	MedicalFinding	preclinical activity against			NULL		0	NULL	NULL	NULL	NULL	NULL	An investigational drug, MLN8237 is an orally available, potent, and selective AAK inhibitor. It has shown preclinical activity against leukemia, lymphoma,	topic_ll
77275	3	355887	7	NULL	NULL	0	NULL	statement 1	Process		shows 					lymphoma	MedicalFinding	preclinical activity against			NULL		0	NULL	NULL	NULL	NULL	NULL	An investigational drug, MLN8237 is an orally available, potent, and selective AAK inhibitor. It has shown preclinical activity against leukemia, lymphoma,	topic_ll
77276	4	355887	7	NULL	NULL	0	NULL	MLN8237	Chemical		is a type of					orally available drug	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	An investigational drug, MLN8237 is an orally available, potent, and selective AAK inhibitor. It has shown preclinical activity against leukemia, lymphoma,	topic_ll
77277	1	355888	7	NULL	NULL	0	NULL	T-rapa cell	Cell		is a type of					white blood cell	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	The T-rapa cell is a type of white blood cell that is cultured with rapamycin, co-stimulation and interleukin-4. These cells express a balanced Th2/Th1 effector phenotype -- a T-cell profile that is thought to protect against transplant rejection and improve the outcome of patients by reducing graft versus host disease and improving graft versus tumor effect.	topic_ll
77278	2	355888	7	NULL	NULL	0	NULL	T-rapa cell	Cell		express					Th2/Th1 effector phenotype	PhysicalPhenomenon	balanced			NULL		0	NULL	NULL	NULL	NULL	NULL	The T-rapa cell is a type of white blood cell that is cultured with rapamycin, co-stimulation and interleukin-4. These cells express a balanced Th2/Th1 effector phenotype -- a T-cell profile that is thought to protect against transplant rejection and improve the outcome of patients by reducing graft versus host disease and improving graft versus tumor effect.	topic_ll
77279	3	355888	7	NULL	NULL	0	NULL	Th2/Th1 effector phenotype	PhysicalPhenomenon		is a type of					T-cell profile	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The T-rapa cell is a type of white blood cell that is cultured with rapamycin, co-stimulation and interleukin-4. These cells express a balanced Th2/Th1 effector phenotype -- a T-cell profile that is thought to protect against transplant rejection and improve the outcome of patients by reducing graft versus host disease and improving graft versus tumor effect.	topic_ll
77280	4	355888	7	NULL	NULL	0	NULL	Th2/Th1 effector phenotype	PhysicalPhenomenon		protect against					transplant rejection	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The T-rapa cell is a type of white blood cell that is cultured with rapamycin, co-stimulation and interleukin-4. These cells express a balanced Th2/Th1 effector phenotype -- a T-cell profile that is thought to protect against transplant rejection and improve the outcome of patients by reducing graft versus host disease and improving graft versus tumor effect.	topic_ll
77281	5	355888	7	NULL	NULL	0	NULL	Th2/Th1 effector phenotype	PhysicalPhenomenon		reduce					graft versus host disease	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The T-rapa cell is a type of white blood cell that is cultured with rapamycin, co-stimulation and interleukin-4. These cells express a balanced Th2/Th1 effector phenotype -- a T-cell profile that is thought to protect against transplant rejection and improve the outcome of patients by reducing graft versus host disease and improving graft versus tumor effect.	topic_ll
77282	6	355888	7	NULL	NULL	0	NULL	Th2/Th1 effector phenotype	PhysicalPhenomenon		improve					graft versus tumor effect	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The T-rapa cell is a type of white blood cell that is cultured with rapamycin, co-stimulation and interleukin-4. These cells express a balanced Th2/Th1 effector phenotype -- a T-cell profile that is thought to protect against transplant rejection and improve the outcome of patients by reducing graft versus host disease and improving graft versus tumor effect.	topic_ll
77283	7	355888	7	NULL	NULL	0	NULL	Th2/Th1 effector phenotype	PhysicalPhenomenon		improve					patients	GroupOfPeople	outcome of			NULL		0	NULL	NULL	NULL	NULL	NULL	The T-rapa cell is a type of white blood cell that is cultured with rapamycin, co-stimulation and interleukin-4. These cells express a balanced Th2/Th1 effector phenotype -- a T-cell profile that is thought to protect against transplant rejection and improve the outcome of patients by reducing graft versus host disease and improving graft versus tumor effect.	topic_ll
77284	8	355888	7	NULL	NULL	0	NULL	statement 7	Process		occur by					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The T-rapa cell is a type of white blood cell that is cultured with rapamycin, co-stimulation and interleukin-4. These cells express a balanced Th2/Th1 effector phenotype -- a T-cell profile that is thought to protect against transplant rejection and improve the outcome of patients by reducing graft versus host disease and improving graft versus tumor effect.	topic_ll
77285	9	355888	7	NULL	NULL	0	NULL	statement 7	Process		occur by					statement 6	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The T-rapa cell is a type of white blood cell that is cultured with rapamycin, co-stimulation and interleukin-4. These cells express a balanced Th2/Th1 effector phenotype -- a T-cell profile that is thought to protect against transplant rejection and improve the outcome of patients by reducing graft versus host disease and improving graft versus tumor effect.	topic_ll
77286	1	355889	7	NULL	NULL	0	NULL	IDH1	GP	mutation of	generate					poison	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	They went on to show that IDH1 and IDH2 mutations generate a 'poison' that blocks the ability of a protective factor called TET2 to remove the methylation from the genome. Interestingly, the researchers also showed that many AML patients have mutations that inactivate TET2, and this causes the same abnormal DNA methylation effect as IDH1 and IDH2 mutations.	topic_ll
77287	3	355889	7	NULL	NULL	NULL	NULL	statement 1	Process		blocks					statement 2	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	They went on to show that IDH1 and IDH2 mutations generate a 'poison' that blocks the ability of a protective factor called TET2 to remove the methylation from the genome. Interestingly, the researchers also showed that many AML patients have mutations that inactivate TET2, and this causes the same abnormal DNA methylation effect as IDH1 and IDH2 mutations.	topic_ll
77288	2	355889	7	NULL	NULL	0	NULL	TET2	GP		remove					genome	Organism	methylation from			NULL		0	NULL	NULL	NULL	NULL	NULL	They went on to show that IDH1 and IDH2 mutations generate a 'poison' that blocks the ability of a protective factor called TET2 to remove the methylation from the genome. Interestingly, the researchers also showed that many AML patients have mutations that inactivate TET2, and this causes the same abnormal DNA methylation effect as IDH1 and IDH2 mutations.	topic_ll
77289	4	355889	7	NULL	NULL	NULL	NULL	AML patients	GroupOfPeople	mutations of	inactivate					TET2	GP				NULL		NULL	NULL	NULL	NULL	NULL	NULL	They went on to show that IDH1 and IDH2 mutations generate a 'poison' that blocks the ability of a protective factor called TET2 to remove the methylation from the genome. Interestingly, the researchers also showed that many AML patients have mutations that inactivate TET2, and this causes the same abnormal DNA methylation effect as IDH1 and IDH2 mutations.	topic_ll
77290	5	355889	7	NULL	NULL	0	NULL	statement 4	Process		cause					IDH1	GP	mutations of			NULL		0	NULL	NULL	NULL	NULL	NULL	They went on to show that IDH1 and IDH2 mutations generate a 'poison' that blocks the ability of a protective factor called TET2 to remove the methylation from the genome. Interestingly, the researchers also showed that many AML patients have mutations that inactivate TET2, and this causes the same abnormal DNA methylation effect as IDH1 and IDH2 mutations.	topic_ll
77291	6	355889	7	NULL	NULL	0	NULL	statement 4	Process		cause					IDH2	GP	mutations of			NULL		0	NULL	NULL	NULL	NULL	NULL	They went on to show that IDH1 and IDH2 mutations generate a 'poison' that blocks the ability of a protective factor called TET2 to remove the methylation from the genome. Interestingly, the researchers also showed that many AML patients have mutations that inactivate TET2, and this causes the same abnormal DNA methylation effect as IDH1 and IDH2 mutations.	topic_ll
77292	7	355889	7	NULL	NULL	0	NULL	IDH1	GP	mutations of	is a type of					abnormal DNA methylation effect	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	They went on to show that IDH1 and IDH2 mutations generate a 'poison' that blocks the ability of a protective factor called TET2 to remove the methylation from the genome. Interestingly, the researchers also showed that many AML patients have mutations that inactivate TET2, and this causes the same abnormal DNA methylation effect as IDH1 and IDH2 mutations.	topic_ll
77293	8	355889	7	NULL	NULL	0	NULL	IDH2	GP	mutations of	generate					poison	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	They went on to show that IDH1 and IDH2 mutations generate a 'poison' that blocks the ability of a protective factor called TET2 to remove the methylation from the genome. Interestingly, the researchers also showed that many AML patients have mutations that inactivate TET2, and this causes the same abnormal DNA methylation effect as IDH1 and IDH2 mutations.	topic_ll
77294	9	355889	7	NULL	NULL	0	NULL	statement 8	Process		blocks					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	They went on to show that IDH1 and IDH2 mutations generate a 'poison' that blocks the ability of a protective factor called TET2 to remove the methylation from the genome. Interestingly, the researchers also showed that many AML patients have mutations that inactivate TET2, and this causes the same abnormal DNA methylation effect as IDH1 and IDH2 mutations.	topic_ll
77295	10	355889	7	NULL	NULL	0	NULL	IDH2	GP	mutations of	is a type of					abnormal DNA methylation effect	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	They went on to show that IDH1 and IDH2 mutations generate a 'poison' that blocks the ability of a protective factor called TET2 to remove the methylation from the genome. Interestingly, the researchers also showed that many AML patients have mutations that inactivate TET2, and this causes the same abnormal DNA methylation effect as IDH1 and IDH2 mutations.	topic_ll
77324	11	355889	7	NULL	NULL	0	NULL	TET2	GP		is a type of					protective factor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	They went on to show that IDH1 and IDH2 mutations generate a 'poison' that blocks the ability of a protective factor called TET2 to remove the methylation from the genome. Interestingly, the researchers also showed that many AML patients have mutations that inactivate TET2, and this causes the same abnormal DNA methylation effect as IDH1 and IDH2 mutations.	topic_ll
77296	1	355891	7	NULL	NULL	0	NULL	AML patients	MedicalFinding	mutations of	inactivate					TET2	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	many AML patients have mutations that inactivate TET2, 	topic_ll
77297	1	355892	7	NULL	NULL	0	NULL	miR-125b	GP	overexpression of	cause		independently			leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Whitehead Institute researchers have shown in mouse models that overexpression of the microRNA 125b (miR-125b) can independently cause leukemia and accelerate the disease's progression.	topic_ll
77298	2	355892	7	NULL	NULL	0	NULL	statement 1	Process		accelerate					disease progression	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Whitehead Institute researchers have shown in mouse models that overexpression of the microRNA 125b (miR-125b) can independently cause leukemia and accelerate the disease's progression.	topic_ll
77299	3	355892	7	NULL	NULL	0	NULL	miR-125b	GP		is					microRNA 125b	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Whitehead Institute researchers have shown in mouse models that overexpression of the microRNA 125b (miR-125b) can independently cause leukemia and accelerate the disease's progression.	topic_ll
77300	1	355893	7	NULL	NULL	NULL	NULL	 ponatinib	Chemical		produce					 hematologic response	Process	complete			NULL		NULL	NULL	NULL	NULL	NULL	NULL	n a Phase I clinical trial, the drug ponatinib produced major or complete hematologic responses (absence of CML cells in the blood) and cytogenetic responses (absence of leukemia cells in the bone marrow) among two groups of patients:	topic_ll
77301	2	355893	7	NULL	NULL	0	NULL	 ponatinib 	Chemical		produce					cytogenetic response	Process	complete			NULL		0	NULL	NULL	NULL	NULL	NULL	n a Phase I clinical trial, the drug ponatinib produced major or complete hematologic responses (absence of CML cells in the blood) and cytogenetic responses (absence of leukemia cells in the bone marrow) among two groups of patients:	topic_ll
77302	3	355893	7	NULL	NULL	0	NULL	hematologic response	Process		is					CML cells	Cell	absence of			NULL		0	NULL	NULL	NULL	NULL	NULL	n a Phase I clinical trial, the drug ponatinib produced major or complete hematologic responses (absence of CML cells in the blood) and cytogenetic responses (absence of leukemia cells in the bone marrow) among two groups of patients:	topic_ll
77303	4	355893	7	NULL	NULL	0	NULL	statement 3	Process		occur in					blood	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	n a Phase I clinical trial, the drug ponatinib produced major or complete hematologic responses (absence of CML cells in the blood) and cytogenetic responses (absence of leukemia cells in the bone marrow) among two groups of patients:	topic_ll
77304	5	355893	7	NULL	NULL	0	NULL	cytogenetic response	Process		is					leukemia cells	Cell	absence of			NULL		0	NULL	NULL	NULL	NULL	NULL	n a Phase I clinical trial, the drug ponatinib produced major or complete hematologic responses (absence of CML cells in the blood) and cytogenetic responses (absence of leukemia cells in the bone marrow) among two groups of patients:	topic_ll
77305	6	355893	7	NULL	NULL	0	NULL	statement 5	Process		occur in					bone marrow	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	n a Phase I clinical trial, the drug ponatinib produced major or complete hematologic responses (absence of CML cells in the blood) and cytogenetic responses (absence of leukemia cells in the bone marrow) among two groups of patients:	topic_ll
77306	1	355894	7	NULL	NULL	0	NULL	ponatinib	Chemical		produce					hematologic response	Process	complete			NULL		0	NULL	NULL	NULL	NULL	NULL	n a Phase I clinical trial, the drug ponatinib produced major or complete hematologic responses (absence of CML cells in the blood) and cytogenetic responses (absence of leukemia cells in the bone marrow) among two groups of patients: And those whose leukemia cells carry the T315I mutation, which resists all current therapies.	topic_ll
77307	2	355894	7	NULL	NULL	NULL	NULL	ponatinib	Chemical		produce					cytogenetic response	Process	complete			NULL		NULL	NULL	NULL	NULL	NULL	NULL	n a Phase I clinical trial, the drug ponatinib produced major or complete hematologic responses (absence of CML cells in the blood) and cytogenetic responses (absence of leukemia cells in the bone marrow) among two groups of patients: And those whose leukemia cells carry the T315I mutation, which resists all current therapies.	topic_ll
77308	3	355894	7	NULL	NULL	0	NULL	hematologic response	Process		is					CML cells	Cell	absence of			NULL		0	NULL	NULL	NULL	NULL	NULL	n a Phase I clinical trial, the drug ponatinib produced major or complete hematologic responses (absence of CML cells in the blood) and cytogenetic responses (absence of leukemia cells in the bone marrow) among two groups of patients: And those whose leukemia cells carry the T315I mutation, which resists all current therapies.	topic_ll
77309	4	355894	7	NULL	NULL	0	NULL	statement 3	Process		occur in					blood	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	n a Phase I clinical trial, the drug ponatinib produced major or complete hematologic responses (absence of CML cells in the blood) and cytogenetic responses (absence of leukemia cells in the bone marrow) among two groups of patients: And those whose leukemia cells carry the T315I mutation, which resists all current therapies.	topic_ll
77310	5	355894	7	NULL	NULL	0	NULL	cytogenetic response	Process		is					leukemia cells	Cell	absence of			NULL		0	NULL	NULL	NULL	NULL	NULL	n a Phase I clinical trial, the drug ponatinib produced major or complete hematologic responses (absence of CML cells in the blood) and cytogenetic responses (absence of leukemia cells in the bone marrow) among two groups of patients: And those whose leukemia cells carry the T315I mutation, which resists all current therapies.	topic_ll
77311	6	355894	7	NULL	NULL	0	NULL	statement 5	Process		occur in					bone marrow	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	n a Phase I clinical trial, the drug ponatinib produced major or complete hematologic responses (absence of CML cells in the blood) and cytogenetic responses (absence of leukemia cells in the bone marrow) among two groups of patients: And those whose leukemia cells carry the T315I mutation, which resists all current therapies.	topic_ll
77312	7	355894	7	NULL	NULL	0	NULL	 leukemia cells	Cell		carry							mutations of	T315I		NULL		0	NULL	NULL	NULL	NULL	NULL	n a Phase I clinical trial, the drug ponatinib produced major or complete hematologic responses (absence of CML cells in the blood) and cytogenetic responses (absence of leukemia cells in the bone marrow) among two groups of patients: And those whose leukemia cells carry the T315I mutation, which resists all current therapies.	topic_ll
77313	8	355894	7	NULL	NULL	0	NULL	statement 7	Process		resist					 therapies	MedicalProcedure	current			NULL		0	NULL	NULL	NULL	NULL	NULL	n a Phase I clinical trial, the drug ponatinib produced major or complete hematologic responses (absence of CML cells in the blood) and cytogenetic responses (absence of leukemia cells in the bone marrow) among two groups of patients: And those whose leukemia cells carry the T315I mutation, which resists all current therapies.	topic_ll
77314	1	355895	7	NULL	NULL	0	NULL	leukemia cells	Cell		carry							mutations of	T315I		NULL		0	NULL	NULL	NULL	NULL	NULL	And those whose leukemia cells carry the T315I mutation, which resists all current therapies.	topic_ll
77315	1	355896	7	NULL	NULL	0	NULL	 leukemia cells	Cell		trigger					protective response	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Massey researchers have uncovered the mechanism by which leukemia cells trigger a protective response when exposed to a class of cancer-killing agents known as histone deacetylase inhibitors (HDACIs). Massey researchers discovered was that HDACIs initially induce DNA damage within the cell nucleus, leading to modification of the NEMO protein, which then triggers the cytoprotective NF-κB pathway. 	topic_ll
77316	2	355896	7	NULL	NULL	0	NULL	statement 1	Process		occur when					HDACIs	Chemical	exposed to			NULL		0	NULL	NULL	NULL	NULL	NULL	Massey researchers have uncovered the mechanism by which leukemia cells trigger a protective response when exposed to a class of cancer-killing agents known as histone deacetylase inhibitors (HDACIs). Massey researchers discovered was that HDACIs initially induce DNA damage within the cell nucleus, leading to modification of the NEMO protein, which then triggers the cytoprotective NF-κB pathway. 	topic_ll
77317	3	355896	7	NULL	NULL	0	NULL	HDACIs	Chemical		is					 histone deacetylase inhibitors	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Massey researchers have uncovered the mechanism by which leukemia cells trigger a protective response when exposed to a class of cancer-killing agents known as histone deacetylase inhibitors (HDACIs). Massey researchers discovered was that HDACIs initially induce DNA damage within the cell nucleus, leading to modification of the NEMO protein, which then triggers the cytoprotective NF-κB pathway. 	topic_ll
77318	4	355896	7	NULL	NULL	0	NULL	HDACIs	Chemical		is a type of					cancer-killing agents	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Massey researchers have uncovered the mechanism by which leukemia cells trigger a protective response when exposed to a class of cancer-killing agents known as histone deacetylase inhibitors (HDACIs). Massey researchers discovered was that HDACIs initially induce DNA damage within the cell nucleus, leading to modification of the NEMO protein, which then triggers the cytoprotective NF-κB pathway. 	topic_ll
77319	5	355896	7	NULL	NULL	0	NULL	HDACIs	Chemical		induce		initially			DNA damage	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Massey researchers have uncovered the mechanism by which leukemia cells trigger a protective response when exposed to a class of cancer-killing agents known as histone deacetylase inhibitors (HDACIs). Massey researchers discovered was that HDACIs initially induce DNA damage within the cell nucleus, leading to modification of the NEMO protein, which then triggers the cytoprotective NF-κB pathway. 	topic_ll
77320	6	355896	7	NULL	NULL	0	NULL	statement 5	Process		occur within					cell nucleus	CellComponent				NULL		0	NULL	NULL	NULL	NULL	NULL	Massey researchers have uncovered the mechanism by which leukemia cells trigger a protective response when exposed to a class of cancer-killing agents known as histone deacetylase inhibitors (HDACIs). Massey researchers discovered was that HDACIs initially induce DNA damage within the cell nucleus, leading to modification of the NEMO protein, which then triggers the cytoprotective NF-κB pathway. 	topic_ll
77321	7	355896	7	NULL	NULL	0	NULL	statement 5	Process		leads to					NEMO protein	GP	modification of			NULL		0	NULL	NULL	NULL	NULL	NULL	Massey researchers have uncovered the mechanism by which leukemia cells trigger a protective response when exposed to a class of cancer-killing agents known as histone deacetylase inhibitors (HDACIs). Massey researchers discovered was that HDACIs initially induce DNA damage within the cell nucleus, leading to modification of the NEMO protein, which then triggers the cytoprotective NF-κB pathway. 	topic_ll
77322	8	355896	7	NULL	NULL	0	NULL	NEMO protein	GP		triggers					 NF-κB pathway	Process	cytoprotective			NULL		0	NULL	NULL	NULL	NULL	NULL	Massey researchers have uncovered the mechanism by which leukemia cells trigger a protective response when exposed to a class of cancer-killing agents known as histone deacetylase inhibitors (HDACIs). Massey researchers discovered was that HDACIs initially induce DNA damage within the cell nucleus, leading to modification of the NEMO protein, which then triggers the cytoprotective NF-κB pathway. 	topic_ll
77325	1	355897	7	NULL	NULL	0	NULL	leukemia cells	Cell		trigger					 protective response	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Massey researchers have uncovered the mechanism by which leukemia cells trigger a protective response when exposed to a class of cancer-killing agents known as histone deacetylase inhibitors (HDACIs).	topic_ll
77326	2	355897	7	NULL	NULL	0	NULL	statement 1	Process		occur when					HDACIs	Chemical	exposed to			NULL		0	NULL	NULL	NULL	NULL	NULL	Massey researchers have uncovered the mechanism by which leukemia cells trigger a protective response when exposed to a class of cancer-killing agents known as histone deacetylase inhibitors (HDACIs).	topic_ll
77327	3	355897	7	NULL	NULL	0	NULL	HDACIs	Chemical		is					histone deacetylase inhibitors	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Massey researchers have uncovered the mechanism by which leukemia cells trigger a protective response when exposed to a class of cancer-killing agents known as histone deacetylase inhibitors (HDACIs).	topic_ll
77328	4	355897	7	NULL	NULL	0	NULL	HDACIs	Chemical		is a type of					cancer-killing agents	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Massey researchers have uncovered the mechanism by which leukemia cells trigger a protective response when exposed to a class of cancer-killing agents known as histone deacetylase inhibitors (HDACIs).	topic_ll
77329	1	355898	7	NULL	NULL	0	NULL	HDACIs	Chemical		induce		initially			DNA damage	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	What VCU Massey researchers discovered was that HDACIs initially induce DNA damage within the cell nucleus, leading to modification of the NEMO protein, which then triggers the cytoprotective NF-κB pathway. By disrupting modifications of the NEMO protein, NF-κB activation can be prevented, and as a consequence, the cancer-killing capacity of HDACIs increases dramatically. NULL	topic_ll
77330	2	355898	7	NULL	NULL	0	NULL	statement 1	Process		occur within					cell nucleus	CellComponent				NULL		0	NULL	NULL	NULL	NULL	NULL	What VCU Massey researchers discovered was that HDACIs initially induce DNA damage within the cell nucleus, leading to modification of the NEMO protein, which then triggers the cytoprotective NF-κB pathway. By disrupting modifications of the NEMO protein, NF-κB activation can be prevented, and as a consequence, the cancer-killing capacity of HDACIs increases dramatically. NULL	topic_ll
77331	3	355898	7	NULL	NULL	0	NULL	statement 1	Process		leads to					NEMO protein	GP	modification of			NULL		0	NULL	NULL	NULL	NULL	NULL	What VCU Massey researchers discovered was that HDACIs initially induce DNA damage within the cell nucleus, leading to modification of the NEMO protein, which then triggers the cytoprotective NF-κB pathway. By disrupting modifications of the NEMO protein, NF-κB activation can be prevented, and as a consequence, the cancer-killing capacity of HDACIs increases dramatically. NULL	topic_ll
77332	4	355898	7	NULL	NULL	0	NULL	NEMO protein	GP		trigger					NF-κB pathway	Process	cytoprotective			NULL		0	NULL	NULL	NULL	NULL	NULL	What VCU Massey researchers discovered was that HDACIs initially induce DNA damage within the cell nucleus, leading to modification of the NEMO protein, which then triggers the cytoprotective NF-κB pathway. By disrupting modifications of the NEMO protein, NF-κB activation can be prevented, and as a consequence, the cancer-killing capacity of HDACIs increases dramatically. NULL	topic_ll
77333	5	355898	7	NULL	NULL	0	NULL	NEMO protein	GP	disrupting modifications of	prevent					NF-κB	GP	activation of			NULL		0	NULL	NULL	NULL	NULL	NULL	What VCU Massey researchers discovered was that HDACIs initially induce DNA damage within the cell nucleus, leading to modification of the NEMO protein, which then triggers the cytoprotective NF-κB pathway. By disrupting modifications of the NEMO protein, NF-κB activation can be prevented, and as a consequence, the cancer-killing capacity of HDACIs increases dramatically. NULL	topic_ll
77334	6	355898	7	NULL	NULL	0	NULL	HDACIs 	Chemical		kills					cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	What VCU Massey researchers discovered was that HDACIs initially induce DNA damage within the cell nucleus, leading to modification of the NEMO protein, which then triggers the cytoprotective NF-κB pathway. By disrupting modifications of the NEMO protein, NF-κB activation can be prevented, and as a consequence, the cancer-killing capacity of HDACIs increases dramatically. NULL	topic_ll
77335	7	355898	7	NULL	NULL	0	NULL	statement 5	Process		increase		dramatically			statement 6	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	What VCU Massey researchers discovered was that HDACIs initially induce DNA damage within the cell nucleus, leading to modification of the NEMO protein, which then triggers the cytoprotective NF-κB pathway. By disrupting modifications of the NEMO protein, NF-κB activation can be prevented, and as a consequence, the cancer-killing capacity of HDACIs increases dramatically. NULL	topic_ll
77336	1	355899	7	NULL	NULL	0	NULL	HDACIs	Chemical		induce		initially			DNA damage	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	What VCU Massey researchers discovered was that HDACIs initially induce DNA damage within the cell nucleus, leading to modification of the NEMO protein, which then triggers the cytoprotective NF-κB pathway. By disrupting modifications of the NEMO protein, NF-κB activation can be prevented, and as a consequence, the cancer-killing capacity of HDACIs increases dramatically. Grant's team is now focusing on ways to capitalize on this discovery by designing strategies that interrupt NEMO modifications through the use of pharmacologic agents and other means. NULL	topic_ll
77337	2	355899	7	NULL	NULL	0	NULL	statement 1	Process		occur within					cell nucleus	CellComponent				NULL		0	NULL	NULL	NULL	NULL	NULL	What VCU Massey researchers discovered was that HDACIs initially induce DNA damage within the cell nucleus, leading to modification of the NEMO protein, which then triggers the cytoprotective NF-κB pathway. By disrupting modifications of the NEMO protein, NF-κB activation can be prevented, and as a consequence, the cancer-killing capacity of HDACIs increases dramatically. Grant's team is now focusing on ways to capitalize on this discovery by designing strategies that interrupt NEMO modifications through the use of pharmacologic agents and other means. NULL	topic_ll
77338	3	355899	7	NULL	NULL	0	NULL	statement 2	Process		leads to					NEMO protein	GP	modification of			NULL		0	NULL	NULL	NULL	NULL	NULL	What VCU Massey researchers discovered was that HDACIs initially induce DNA damage within the cell nucleus, leading to modification of the NEMO protein, which then triggers the cytoprotective NF-κB pathway. By disrupting modifications of the NEMO protein, NF-κB activation can be prevented, and as a consequence, the cancer-killing capacity of HDACIs increases dramatically. Grant's team is now focusing on ways to capitalize on this discovery by designing strategies that interrupt NEMO modifications through the use of pharmacologic agents and other means. NULL	topic_ll
77339	4	355899	7	NULL	NULL	0	NULL	statement 3	Process		trigger					NF-κB pathway	Process	cytoprotective			NULL		0	NULL	NULL	NULL	NULL	NULL	What VCU Massey researchers discovered was that HDACIs initially induce DNA damage within the cell nucleus, leading to modification of the NEMO protein, which then triggers the cytoprotective NF-κB pathway. By disrupting modifications of the NEMO protein, NF-κB activation can be prevented, and as a consequence, the cancer-killing capacity of HDACIs increases dramatically. Grant's team is now focusing on ways to capitalize on this discovery by designing strategies that interrupt NEMO modifications through the use of pharmacologic agents and other means. NULL	topic_ll
77340	5	355899	7	NULL	NULL	0	NULL	NEMO protein	GP	disrupting modifications of	prevents					NF-κB	GP	activation of			NULL		0	NULL	NULL	NULL	NULL	NULL	What VCU Massey researchers discovered was that HDACIs initially induce DNA damage within the cell nucleus, leading to modification of the NEMO protein, which then triggers the cytoprotective NF-κB pathway. By disrupting modifications of the NEMO protein, NF-κB activation can be prevented, and as a consequence, the cancer-killing capacity of HDACIs increases dramatically. Grant's team is now focusing on ways to capitalize on this discovery by designing strategies that interrupt NEMO modifications through the use of pharmacologic agents and other means. NULL	topic_ll
77341	6	355899	7	NULL	NULL	0	NULL	HDACIs 	Chemical		kills					cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	What VCU Massey researchers discovered was that HDACIs initially induce DNA damage within the cell nucleus, leading to modification of the NEMO protein, which then triggers the cytoprotective NF-κB pathway. By disrupting modifications of the NEMO protein, NF-κB activation can be prevented, and as a consequence, the cancer-killing capacity of HDACIs increases dramatically. Grant's team is now focusing on ways to capitalize on this discovery by designing strategies that interrupt NEMO modifications through the use of pharmacologic agents and other means. NULL	topic_ll
77342	7	355899	7	NULL	NULL	0	NULL	statement 5	Process		increase		dramatically			statement 6	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	What VCU Massey researchers discovered was that HDACIs initially induce DNA damage within the cell nucleus, leading to modification of the NEMO protein, which then triggers the cytoprotective NF-κB pathway. By disrupting modifications of the NEMO protein, NF-κB activation can be prevented, and as a consequence, the cancer-killing capacity of HDACIs increases dramatically. Grant's team is now focusing on ways to capitalize on this discovery by designing strategies that interrupt NEMO modifications through the use of pharmacologic agents and other means. NULL	topic_ll
76595	1	355909	5	NULL	NULL	0	NULL	GABAergic system	OrganismPart	hypofunction of	plays a causal role in					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The hypofunction of GABAergic system and glutamate toxicity are generally believed to have a causal role for autism.	topic_aut
76596	2	355909	5	NULL	NULL	0	NULL	glutamate toxicity	MedicalFinding		plays a causal role in					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The hypofunction of GABAergic system and glutamate toxicity are generally believed to have a causal role for autism.	topic_aut
76597	1	355910	5	NULL	NULL	0	NULL	NMDA	Chemical		is					N-methyl-D: -aspartic acid	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The antagonist of the N-methyl-D: -aspartic acid (NMDA) glutamate receptor improves autism. Glycine is required for the activation of NMDA receptor. The antagonist of glycine site decreases NMDA receptor conductance. It is hypothesis that glycine site antagonists can be tested as a new strategy for the management of autism.	topic_aut
76598	2	355910	5	NULL	NULL	0	NULL	(NMDA glutamate receptor antagonist	Chemical		improves					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The antagonist of the N-methyl-D: -aspartic acid (NMDA) glutamate receptor improves autism. Glycine is required for the activation of NMDA receptor. The antagonist of glycine site decreases NMDA receptor conductance. It is hypothesis that glycine site antagonists can be tested as a new strategy for the management of autism.	topic_aut
76599	3	355910	5	NULL	NULL	0	NULL	Glycine	Chemical		activates					NMDA receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The antagonist of the N-methyl-D: -aspartic acid (NMDA) glutamate receptor improves autism. Glycine is required for the activation of NMDA receptor. The antagonist of glycine site decreases NMDA receptor conductance. It is hypothesis that glycine site antagonists can be tested as a new strategy for the management of autism.	topic_aut
76600	4	355910	5	NULL	NULL	0	NULL	glycine site antagonist	Chemical		decreases					NMDA receptor 	GP	conductance of			NULL		0	NULL	NULL	NULL	NULL	NULL	The antagonist of the N-methyl-D: -aspartic acid (NMDA) glutamate receptor improves autism. Glycine is required for the activation of NMDA receptor. The antagonist of glycine site decreases NMDA receptor conductance. It is hypothesis that glycine site antagonists can be tested as a new strategy for the management of autism.	topic_aut
76601	5	355910	5	NULL	NULL	0	NULL	glycine site antagonists	Chemical		plays a role in					autism	MedicalFinding	management of			NULL		0	NULL	NULL	NULL	NULL	NULL	The antagonist of the N-methyl-D: -aspartic acid (NMDA) glutamate receptor improves autism. Glycine is required for the activation of NMDA receptor. The antagonist of glycine site decreases NMDA receptor conductance. It is hypothesis that glycine site antagonists can be tested as a new strategy for the management of autism.	topic_aut
76602	1	355911	5	NULL	NULL	0	NULL	brain membranes	OrganismPart		undergoes					degradation	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The degradation of brain membranes in autism (2) and the role of phospholipases (3) in autism has been reported for many years	topic_aut
76603	2	355911	5	NULL	NULL	0	NULL	statement 1	Process		occurs in					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The degradation of brain membranes in autism (2) and the role of phospholipases (3) in autism has been reported for many years	topic_aut
76604	3	355911	5	NULL	NULL	0	NULL	phospholipases	GP		plays a role in					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The degradation of brain membranes in autism (2) and the role of phospholipases (3) in autism has been reported for many years	topic_aut
76605	1	355914	5	NULL	NULL	0	NULL	memantine	Chemical		is a antagonist of					Glutamate	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamate antagonists (7) such as memantine, an antagonist of the N-methyl-D-aspartic acid (NMDA) glutamate receptor, have shown a significant improvement in open-label use for autism	topic_aut
76606	2	355914	5	NULL	NULL	0	NULL	NMDA	Chemical		is					N-methyl-D-aspartic acid	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamate antagonists (7) such as memantine, an antagonist of the N-methyl-D-aspartic acid (NMDA) glutamate receptor, have shown a significant improvement in open-label use for autism	topic_aut
76607	3	355914	5	NULL	NULL	0	NULL	NMDA glutamate receptor antagonist	Chemical		is used to treat					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamate antagonists (7) such as memantine, an antagonist of the N-methyl-D-aspartic acid (NMDA) glutamate receptor, have shown a significant improvement in open-label use for autism	topic_aut
76608	4	355914	5	NULL	NULL	0	NULL	NMDA glutamate receptor antagonist	Process		is used in					open-label trial	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamate antagonists (7) such as memantine, an antagonist of the N-methyl-D-aspartic acid (NMDA) glutamate receptor, have shown a significant improvement in open-label use for autism	topic_aut
76609	5	355914	5	NULL	NULL	0	NULL	memantine	Chemical		is used to treat					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamate antagonists (7) such as memantine, an antagonist of the N-methyl-D-aspartic acid (NMDA) glutamate receptor, have shown a significant improvement in open-label use for autism	topic_aut
76610	6	355914	5	NULL	NULL	0	NULL	memantine	Chemical		is used in					open-label trial	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamate antagonists (7) such as memantine, an antagonist of the N-methyl-D-aspartic acid (NMDA) glutamate receptor, have shown a significant improvement in open-label use for autism	topic_aut
76611	1	355915	5	NULL	NULL	0	NULL	proinflammatory cytokines	GP	enhanced	is observed in					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Enhanced proinflammatory cytokines and activation of microglia and astrocytes are observed in autism	topic_aut
76612	2	355915	5	NULL	NULL	0	NULL	microglia	Cell		is activated in					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Enhanced proinflammatory cytokines and activation of microglia and astrocytes are observed in autism	topic_aut
76613	3	355915	5	NULL	NULL	0	NULL	astrocytes	Cell		is activated in					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Enhanced proinflammatory cytokines and activation of microglia and astrocytes are observed in autism	topic_aut
76614	1	355916	5	NULL	NULL	0	NULL	inflammation	MedicalFinding	active	is observed in					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In addition, active inflammation has been noted in autism	topic_aut
76615	1	355917	5	NULL	NULL	0	NULL	IL-1β	GP	enhanced activity of	is associated with					neuroinflammation	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Enhanced IL-1β activity is associated with neuroinflammation	topic_aut
76616	1	355919	5	NULL	NULL	0	NULL	TNF-α	GP		induce					nitric oxide	Chemical				NULL	brain	0	NULL	NULL	NULL	NULL	NULL	TNF-α is neurotoxic and induces nitric oxide and free radicals in the brain. Enhanced IL-1β activity is associated with neuroinflammation (16). Therefore, excessive glutamate enhances proinflammatory activities and induces neurotoxicity.	topic_aut
76617	2	355919	5	NULL	NULL	0	NULL	TNF-α	GP		induce					free radicals	Chemical				NULL	brain	0	NULL	NULL	NULL	NULL	NULL	TNF-α is neurotoxic and induces nitric oxide and free radicals in the brain. Enhanced IL-1β activity is associated with neuroinflammation (16). Therefore, excessive glutamate enhances proinflammatory activities and induces neurotoxicity.	topic_aut
76618	3	355919	5	NULL	NULL	0	NULL	TNF-α	GP		is a type of					neurotoxic	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	TNF-α is neurotoxic and induces nitric oxide and free radicals in the brain. Enhanced IL-1β activity is associated with neuroinflammation (16). Therefore, excessive glutamate enhances proinflammatory activities and induces neurotoxicity.	topic_aut
76619	4	355919	5	NULL	NULL	0	NULL	IL-1β 	GP	enhanced activity of	is associated with					neuroinflammation	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	TNF-α is neurotoxic and induces nitric oxide and free radicals in the brain. Enhanced IL-1β activity is associated with neuroinflammation (16). Therefore, excessive glutamate enhances proinflammatory activities and induces neurotoxicity.	topic_aut
76620	5	355919	5	NULL	NULL	0	NULL	glutamate	Chemical	excessive	enhances					proinflammatory activities	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	TNF-α is neurotoxic and induces nitric oxide and free radicals in the brain. Enhanced IL-1β activity is associated with neuroinflammation (16). Therefore, excessive glutamate enhances proinflammatory activities and induces neurotoxicity.	topic_aut
76621	6	355919	5	NULL	NULL	0	NULL	statement 5	Process		induce					neurotoxicity	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	TNF-α is neurotoxic and induces nitric oxide and free radicals in the brain. Enhanced IL-1β activity is associated with neuroinflammation (16). Therefore, excessive glutamate enhances proinflammatory activities and induces neurotoxicity.	topic_aut
76691	1	355921	5	NULL	NULL	NULL	NULL	glutamate stress	PhysicalPhenomenon		is associated with					phospholipid biomarkers	AbstractConcept	plasma			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Considering that glutamate stress is associated with plasma phospholipid biomarkers	topic_aut
76692	1	355922	5	NULL	NULL	0	NULL	MSO	Chemical		is					methionine sulfoximine	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	It is interesting that another recently published study introduced methionine sulfoximine (MSO) as an inhibitor of glutamine synthetase (17). MSO decreases the glutamate level in the brains of animal models (17). Therefore, MSO may play a role in lowering the level of plasma phospholipid biomarkers in autism.	topic_aut
76693	2	355922	5	NULL	NULL	0	NULL	MSO	Chemical		is an inhibitor of					glutamine synthetase	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	It is interesting that another recently published study introduced methionine sulfoximine (MSO) as an inhibitor of glutamine synthetase (17). MSO decreases the glutamate level in the brains of animal models (17). Therefore, MSO may play a role in lowering the level of plasma phospholipid biomarkers in autism.	topic_aut
76694	3	355922	5	NULL	NULL	0	NULL	MSO	Chemical		decrease					glutamate	Chemical	levels of			NULL		0	NULL	NULL	NULL	NULL	NULL	It is interesting that another recently published study introduced methionine sulfoximine (MSO) as an inhibitor of glutamine synthetase (17). MSO decreases the glutamate level in the brains of animal models (17). Therefore, MSO may play a role in lowering the level of plasma phospholipid biomarkers in autism.	topic_aut
76695	4	355922	5	NULL	NULL	0	NULL	statement 3	Process		occurs in					brain	OrganismPart				NULL	animal models	0	NULL	NULL	NULL	NULL	NULL	It is interesting that another recently published study introduced methionine sulfoximine (MSO) as an inhibitor of glutamine synthetase (17). MSO decreases the glutamate level in the brains of animal models (17). Therefore, MSO may play a role in lowering the level of plasma phospholipid biomarkers in autism.	topic_aut
76696	5	355922	5	NULL	NULL	0	NULL	MSO	Chemical		lowers		possibly			phospholipid biomarkers	AbstractConcept	plasma			NULL		0	NULL	NULL	NULL	NULL	NULL	It is interesting that another recently published study introduced methionine sulfoximine (MSO) as an inhibitor of glutamine synthetase (17). MSO decreases the glutamate level in the brains of animal models (17). Therefore, MSO may play a role in lowering the level of plasma phospholipid biomarkers in autism.	topic_aut
76697	6	355922	5	NULL	NULL	0	NULL	statement 5	Process		occurs in					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	It is interesting that another recently published study introduced methionine sulfoximine (MSO) as an inhibitor of glutamine synthetase (17). MSO decreases the glutamate level in the brains of animal models (17). Therefore, MSO may play a role in lowering the level of plasma phospholipid biomarkers in autism.	topic_aut
76698	1	355924	5	NULL	NULL	0	NULL	Tumor necrosis factor	GP		is a type of					cytokine	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor necrosis factor is a cytokine involved in systemic inflammation	topic_aut
76699	2	355924	5	NULL	NULL	0	NULL	Tumor necrosis factor	GP		is involved in					systemic inflammation	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor necrosis factor is a cytokine involved in systemic inflammation	topic_aut
76700	1	355925	5	NULL	NULL	0	NULL	IL-1β	GP		is					Interleukin-1 beta	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-1 beta (IL-1β) also known as catabolin, is a cytokine protein	topic_aut
76701	2	355925	5	NULL	NULL	0	NULL	Interleukin-1 beta	GP		is also known as					catabolin	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-1 beta (IL-1β) also known as catabolin, is a cytokine protein	topic_aut
76702	3	355925	5	NULL	NULL	0	NULL	Interleukin-1 beta	GP		is a type of					cytokine protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-1 beta (IL-1β) also known as catabolin, is a cytokine protein	topic_aut
76703	1	355926	5	NULL	NULL	0	NULL	PBDE	Chemical		is					Polybrominated diphenyl ethers	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Polybrominated diphenyl ethers or PBDE, are organobromine compounds that are used as flame retardants	topic_aut
76704	2	355926	5	NULL	NULL	0	NULL	PBDE	Chemical		is a type of					organobromine compounds	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Polybrominated diphenyl ethers or PBDE, are organobromine compounds that are used as flame retardants	topic_aut
76705	3	355926	5	NULL	NULL	0	NULL	PBDE	Chemical		is used as					flame retardants	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Polybrominated diphenyl ethers or PBDE, are organobromine compounds that are used as flame retardants	topic_aut
76706	1	355927	5	NULL	NULL	0	NULL	environmental trigger	PhysicalPhenomenon		activates					mast cell	Cell	non-allergic			NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest non-allergic mast cell activation, probably in response to environmental and stress triggers that could contribute to inflammation	topic_aut
76707	2	355927	5	NULL	NULL	0	NULL	stress trigger	PhysicalPhenomenon		activates					mast cell	Cell	non-allergic			NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest non-allergic mast cell activation, probably in response to environmental and stress triggers that could contribute to inflammation	topic_aut
76708	3	355927	5	NULL	NULL	0	NULL	statement 1	Process		contribute to					inflammation	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest non-allergic mast cell activation, probably in response to environmental and stress triggers that could contribute to inflammation	topic_aut
76709	4	355927	5	NULL	NULL	0	NULL	statement 2	Process		contribute to					inflammation	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest non-allergic mast cell activation, probably in response to environmental and stress triggers that could contribute to inflammation	topic_aut
76710	1	355928	5	NULL	NULL	0	NULL	utero	OrganismPart	inflammation of	leads to					labor	PhysicalPhenomenon	preterm			NULL		0	NULL	NULL	NULL	NULL	NULL	In utero inflammation can lead to preterm labor and has itself been strongly associated with adverse neurodevelopmental outcomes.	topic_aut
76711	2	355928	5	NULL	NULL	0	NULL	statement 2			is associated with		strongly			neurodevelopmental outcomes	MedicalFinding	adverse			NULL		0	NULL	NULL	NULL	NULL	NULL	In utero inflammation can lead to preterm labor and has itself been strongly associated with adverse neurodevelopmental outcomes.	topic_aut
76712	1	355929	5	NULL	NULL	0	NULL	SERT	GP		is					serotonin transporter	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The known Gly56Ala mutation in the serotonin transporter SERT (or 5-HTT), encoded by the SLC6A4 gene, causes increased serotonin reuptake and has been associated with autism and rigid-compulsive behavior	topic_aut
76713	2	355929	5	NULL	NULL	0	NULL	SERT	GP		is also known as					5-HTT	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The known Gly56Ala mutation in the serotonin transporter SERT (or 5-HTT), encoded by the SLC6A4 gene, causes increased serotonin reuptake and has been associated with autism and rigid-compulsive behavior	topic_aut
76714	3	355929	5	NULL	NULL	0	NULL	SERT	GP		is encoded by					SLC6A4 gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The known Gly56Ala mutation in the serotonin transporter SERT (or 5-HTT), encoded by the SLC6A4 gene, causes increased serotonin reuptake and has been associated with autism and rigid-compulsive behavior	topic_aut
76715	4	355929	5	NULL	NULL	0	NULL	SERT	GP	mutant	increases			Gly56Ala		serotonin	Chemical	uptake of			NULL		0	NULL	NULL	NULL	NULL	NULL	The known Gly56Ala mutation in the serotonin transporter SERT (or 5-HTT), encoded by the SLC6A4 gene, causes increased serotonin reuptake and has been associated with autism and rigid-compulsive behavior	topic_aut
76716	5	355929	5	NULL	NULL	0	NULL	SERT	GP	mutant	is associated with			Gly56Ala		autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The known Gly56Ala mutation in the serotonin transporter SERT (or 5-HTT), encoded by the SLC6A4 gene, causes increased serotonin reuptake and has been associated with autism and rigid-compulsive behavior	topic_aut
76717	6	355929	5	NULL	NULL	0	NULL	SERT	GP	mutant	is associated with			Gly56Ala		rigid-compulsive behavior	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The known Gly56Ala mutation in the serotonin transporter SERT (or 5-HTT), encoded by the SLC6A4 gene, causes increased serotonin reuptake and has been associated with autism and rigid-compulsive behavior	topic_aut
76718	1	355930	5	NULL	NULL	0	NULL	SERT	GP		is					serotonin transporter	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The serotonin transporter (SERT) is a monoamine transporter protein.	topic_aut
76719	2	355930	5	NULL	NULL	0	NULL	SERT	GP		is a type of					monoamine transporter protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The serotonin transporter (SERT) is a monoamine transporter protein.	topic_aut
76720	1	355931	5	NULL	NULL	0	NULL	5HIAA	Chemical		is					5-hydroxyindolacetic acid	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Low levels of the serotonin end-metabolite 5-hydroxyindolacetic acid (5HIAA) in CSF were detected	topic_aut
76721	2	355931	5	NULL	NULL	0	NULL	5HIAA	Chemical		is an end-metabolite of					serotonin	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Low levels of the serotonin end-metabolite 5-hydroxyindolacetic acid (5HIAA) in CSF were detected	topic_aut
76722	3	355931	5	NULL	NULL	0	NULL	CSF	OrganismPart		contains					5HIAA	Chemical	low levels of			NULL		0	NULL	NULL	NULL	NULL	NULL	Low levels of the serotonin end-metabolite 5-hydroxyindolacetic acid (5HIAA) in CSF were detected	topic_aut
76723	1	355933	5	NULL	NULL	0	NULL	MAO	GP		is					Monoamine oxidases	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Monoamine oxidases (MAO) (EC 1.4.3.4) are a family of enzymes that catalyze the oxidation of monoamines	topic_aut
76724	2	355933	5	NULL	NULL	0	NULL	MAO	GP		is a family of					enzymes	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Monoamine oxidases (MAO) (EC 1.4.3.4) are a family of enzymes that catalyze the oxidation of monoamines	topic_aut
76725	3	355933	5	NULL	NULL	0	NULL	MAO	GP		oxidize					monoamines	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Monoamine oxidases (MAO) (EC 1.4.3.4) are a family of enzymes that catalyze the oxidation of monoamines	topic_aut
76726	1	355934	5	NULL	NULL	0	NULL	Shank3	GP		plays a role in		important			synaptic function	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 Our results are consistent with altered synaptic development and function in Shank3 haploinsufficiency, highlighting the importance of Shank3 in synaptic function and supporting a link between deficits in synapse function and neurodevelopmental disorders	topic_aut
76727	2	355934	5	NULL	NULL	0	NULL	synapse function	Process	deficits of	is linked to					neurodevelopmental disorders	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	 Our results are consistent with altered synaptic development and function in Shank3 haploinsufficiency, highlighting the importance of Shank3 in synaptic function and supporting a link between deficits in synapse function and neurodevelopmental disorders	topic_aut
76728	3	355934	5	NULL	NULL	0	NULL	Shank3	GP		plays a role in		important			statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 Our results are consistent with altered synaptic development and function in Shank3 haploinsufficiency, highlighting the importance of Shank3 in synaptic function and supporting a link between deficits in synapse function and neurodevelopmental disorders	topic_aut
76729	1	355935	5	NULL	NULL	0	NULL	IBI	MedicalProcedure		is					Intensive Behavioural Intervention	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence-based treatments such as behavioural therapies, have come to the forefront of autism literature Smith (1999), in his review of outcome studies, recognized Intensive Behavioural Intervention (IBI) as the most effective treatment for autism	topic_aut
76730	2	355935	5	NULL	NULL	0	NULL	Intensive Behavioural Intervention	MedicalProcedure		is treatment for		most effective			autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence-based treatments such as behavioural therapies, have come to the forefront of autism literature Smith (1999), in his review of outcome studies, recognized Intensive Behavioural Intervention (IBI) as the most effective treatment for autism	topic_aut
76731	1	355936	5	NULL	NULL	0	NULL	Secretin	GP		does not play a role in					ASD	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	Secretin was an unstudied treatment that gained widespread popularity and use through anecdotal reports before scientific investigation failed to find any evidence of efficacy for treating ASD	topic_aut
76732	1	355937	5	NULL	NULL	0	NULL	Secretin	GP		is a type of					gastrointestinal hormone	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Secretin is a gastrointestinal hormone that stimulates the secretion of bile from the liver, as well as acts as a stress regulatory hormone that impacts GABA levels	topic_aut
76733	2	355937	5	NULL	NULL	0	NULL	bile	OrganismPart		is secreted from					liver	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Secretin is a gastrointestinal hormone that stimulates the secretion of bile from the liver, as well as acts as a stress regulatory hormone that impacts GABA levels	topic_aut
76734	3	355937	5	NULL	NULL	0	NULL	Secretin	GP		stimulates					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Secretin is a gastrointestinal hormone that stimulates the secretion of bile from the liver, as well as acts as a stress regulatory hormone that impacts GABA levels	topic_aut
76735	4	355937	5	NULL	NULL	0	NULL	Secretin	GP		act as					stress regulatory hormone	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Secretin is a gastrointestinal hormone that stimulates the secretion of bile from the liver, as well as acts as a stress regulatory hormone that impacts GABA levels	topic_aut
76736	5	355937	5	NULL	NULL	0	NULL	statement 4	Process		impacts					GABA	Chemical	level of			NULL		0	NULL	NULL	NULL	NULL	NULL	Secretin is a gastrointestinal hormone that stimulates the secretion of bile from the liver, as well as acts as a stress regulatory hormone that impacts GABA levels	topic_aut
76737	1	355938	5	NULL	NULL	0	NULL	GABA receptors	GP		is a class of					receptors	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The GABA receptors are a class of receptors that respond to the neurotransmitter gamma-aminobutyric acid (GABA)	topic_aut
76738	2	355938	5	NULL	NULL	NULL	NULL	GABA receptors	GP		respond to					GABA	Chemical				NULL		NULL	NULL	NULL	NULL	NULL	NULL	The GABA receptors are a class of receptors that respond to the neurotransmitter gamma-aminobutyric acid (GABA)	topic_aut
76739	3	355938	5	NULL	NULL	0	NULL	GABA	Chemical		is					gamma-aminobutyric acid	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The GABA receptors are a class of receptors that respond to the neurotransmitter gamma-aminobutyric acid (GABA)	topic_aut
76740	4	355938	5	NULL	NULL	0	NULL	GABA	Chemical		is a type of					neurotransmitter	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The GABA receptors are a class of receptors that respond to the neurotransmitter gamma-aminobutyric acid (GABA)	topic_aut
76741	1	355939	5	NULL	NULL	0	NULL	alternative diets	Food		does not play a role in					ASD	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	There is little to no empirical support for alternative diets in treating ASD	topic_aut
76742	1	355941	5	NULL	NULL	0	NULL	Martin??Bell syndrome	MedicalFinding		is also known as					Fragile X syndrome	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Fragile X syndrome or Martin–Bell syndrome, is a genetic syndrome	topic_aut
76743	2	355941	5	NULL	NULL	0	NULL	Martin??Bell syndrome	MedicalFinding		is a type of					genetic syndrome	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Fragile X syndrome or Martin–Bell syndrome, is a genetic syndrome	topic_aut
76744	1	355942	5	NULL	NULL	0	NULL	INN	Chemical		is					Thiomersal	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Thiomersal (INN) and commonly known in the US as thimerosal, is an organomercury compound.	topic_aut
76745	2	355942	5	NULL	NULL	0	NULL	Thiomersal	Chemical		is commonly known as					thimerosal	Chemical				NULL	US	0	NULL	NULL	NULL	NULL	NULL	Thiomersal (INN) and commonly known in the US as thimerosal, is an organomercury compound.	topic_aut
76746	3	355942	5	NULL	NULL	0	NULL	INN	Chemical		is a type of					organomercury compound	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Thiomersal (INN) and commonly known in the US as thimerosal, is an organomercury compound.	topic_aut
76747	1	355943	5	NULL	NULL	0	NULL	CD38	GP		is					cluster of differentiation 38	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	CD38 (cluster of differentiation 38), also known as cyclic ADP ribose hydrolase is a glycoprotein[1] found on the surface of many immune cells 	topic_aut
76748	2	355943	5	NULL	NULL	0	NULL	CD38	GP		is also known as					cyclic ADP ribose hydrolase	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	CD38 (cluster of differentiation 38), also known as cyclic ADP ribose hydrolase is a glycoprotein[1] found on the surface of many immune cells 	topic_aut
76749	3	355943	5	NULL	NULL	0	NULL	CD38	GP		is a type of					glycoprotein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	CD38 (cluster of differentiation 38), also known as cyclic ADP ribose hydrolase is a glycoprotein[1] found on the surface of many immune cells 	topic_aut
76750	4	355943	5	NULL	NULL	0	NULL	CD38	GP		is found on					immune cells	Cell	surface of			NULL		0	NULL	NULL	NULL	NULL	NULL	CD38 (cluster of differentiation 38), also known as cyclic ADP ribose hydrolase is a glycoprotein[1] found on the surface of many immune cells 	topic_aut
76751	1	355944	5	NULL	NULL	0	NULL	uridine phosphorylase	GP		is a type of					enzyme	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	In enzymology, an uridine phosphorylase (EC 2.4.2.3) is an enzyme	topic_aut
76752	1	355945	5	NULL	NULL	0	NULL	5-HIAA	Chemical		is					5-Hydroxyindoleacetic acid	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	5-Hydroxyindoleacetic acid (5-HIAA) is the main metabolite of serotonin in the human body	topic_aut
76753	2	355945	5	NULL	NULL	0	NULL	5-HIAA	Chemical		is a metabolite of					serotonin	Chemical				NULL	human body	0	NULL	NULL	NULL	NULL	NULL	5-Hydroxyindoleacetic acid (5-HIAA) is the main metabolite of serotonin in the human body	topic_aut
76754	1	355946	5	NULL	NULL	0	NULL	VNTR	Chromosome		is					Variable Number Tandem Repeat	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	A Variable Number Tandem Repeat (or VNTR) is a location in a genome where a short nucleotide sequence is organized as a tandem repeat	topic_aut
76755	2	355946	5	NULL	NULL	0	NULL	VNTR	Chromosome		is located on					genome	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	A Variable Number Tandem Repeat (or VNTR) is a location in a genome where a short nucleotide sequence is organized as a tandem repeat	topic_aut
76756	3	355946	5	NULL	NULL	0	NULL	nucleotide sequence	NucleicAcid	short	is organized as					tandem repeat	NucleicAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	A Variable Number Tandem Repeat (or VNTR) is a location in a genome where a short nucleotide sequence is organized as a tandem repeat	topic_aut
76757	4	355946	5	NULL	NULL	0	NULL	statement 3	Process		forms					VNTR	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	A Variable Number Tandem Repeat (or VNTR) is a location in a genome where a short nucleotide sequence is organized as a tandem repeat	topic_aut
76758	1	355947	5	NULL	NULL	0	NULL	β-blockers	Chemical		is					Beta blockers	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Beta blockers (sometimes written as β-blockers) or beta-adrenergic blocking agents, beta-adrenergic antagonists, or beta antagonists, are a class of drugs used for various indications, but particularly for the management of cardiac arrhythmias, cardioprotection after myocardial infarction	topic_aut
76759	2	355947	5	NULL	NULL	0	NULL	Beta blockers	Chemical		is also known as					 beta-adrenergic blocking agents	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Beta blockers (sometimes written as β-blockers) or beta-adrenergic blocking agents, beta-adrenergic antagonists, or beta antagonists, are a class of drugs used for various indications, but particularly for the management of cardiac arrhythmias, cardioprotection after myocardial infarction	topic_aut
76760	3	355947	5	NULL	NULL	0	NULL	Beta blockers	Chemical		is also known as					beta-adrenergic antagonists	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Beta blockers (sometimes written as β-blockers) or beta-adrenergic blocking agents, beta-adrenergic antagonists, or beta antagonists, are a class of drugs used for various indications, but particularly for the management of cardiac arrhythmias, cardioprotection after myocardial infarction	topic_aut
76761	4	355947	5	NULL	NULL	0	NULL	Beta blockers	Chemical		is also known as					beta antagonists	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Beta blockers (sometimes written as β-blockers) or beta-adrenergic blocking agents, beta-adrenergic antagonists, or beta antagonists, are a class of drugs used for various indications, but particularly for the management of cardiac arrhythmias, cardioprotection after myocardial infarction	topic_aut
76762	5	355947	5	NULL	NULL	0	NULL	Beta blockers	Chemical		is a class of					drugs	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Beta blockers (sometimes written as β-blockers) or beta-adrenergic blocking agents, beta-adrenergic antagonists, or beta antagonists, are a class of drugs used for various indications, but particularly for the management of cardiac arrhythmias, cardioprotection after myocardial infarction	topic_aut
76763	6	355947	5	NULL	NULL	0	NULL	Beta blockers	Chemical		is used in					cardiac arrhythmias	MedicalFinding	management of			NULL		0	NULL	NULL	NULL	NULL	NULL	Beta blockers (sometimes written as β-blockers) or beta-adrenergic blocking agents, beta-adrenergic antagonists, or beta antagonists, are a class of drugs used for various indications, but particularly for the management of cardiac arrhythmias, cardioprotection after myocardial infarction	topic_aut
76764	7	355947	5	NULL	NULL	0	NULL	Beta blockers	Chemical		is used in					cardioprotection	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Beta blockers (sometimes written as β-blockers) or beta-adrenergic blocking agents, beta-adrenergic antagonists, or beta antagonists, are a class of drugs used for various indications, but particularly for the management of cardiac arrhythmias, cardioprotection after myocardial infarction	topic_aut
76765	8	355947	5	NULL	NULL	0	NULL	statement 7	Process		occurs after					myocardial infarction	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Beta blockers (sometimes written as β-blockers) or beta-adrenergic blocking agents, beta-adrenergic antagonists, or beta antagonists, are a class of drugs used for various indications, but particularly for the management of cardiac arrhythmias, cardioprotection after myocardial infarction	topic_aut
76766	1	355948	5	NULL	NULL	0	NULL	Catecholamines	GP		is a type of					"fight-or-flight" hormones	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Catecholamines are "fight-or-flight" hormones	topic_aut
76767	1	355949	5	NULL	NULL	0	NULL	genomic DNA	NucleicAcid	alterations of	is known as					Copy-number variations	NucleicAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	Copy-number variations are alterations of genomic DNA that correspond to relatively large regions of the genome that have been deleted or amplified on certain chromosomes	topic_aut
76768	1	355950	5	NULL	NULL	0	NULL	Cytokines	GP		is a type of					small cell-signaling protein molecules	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Cytokines (Greek cyto-, cell; and -kinos, movement) are small cell-signaling protein molecules	topic_aut
76769	1	355951	5	NULL	NULL	0	NULL	GABA	Chemical		is					γ-Aminobutyric acid	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	γ-Aminobutyric acid (GABA) is the chief inhibitory neurotransmitter in the mammalian central nervous system	topic_aut
76770	2	355951	5	NULL	NULL	0	NULL	GABA	Chemical		is a type of					 inhibitory neurotransmitter	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	γ-Aminobutyric acid (GABA) is the chief inhibitory neurotransmitter in the mammalian central nervous system	topic_aut
76771	3	355951	5	NULL	NULL	0	NULL	GABA	Chemical		is present in					central nervous system	OrganismPart	mammalian			NULL		0	NULL	NULL	NULL	NULL	NULL	γ-Aminobutyric acid (GABA) is the chief inhibitory neurotransmitter in the mammalian central nervous system	topic_aut
78672	1	355952	11	NULL	NULL	0	NULL	Staphylococcus aureus skin and soft tissue infections	MedicalFinding		is					SSTI	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	This document is intended to provide interim clinical guidance for management of Staphylococcus aureus skin and soft tissue infections (SSTI) in outpatients in Illinois	topic_mrs
78673	1	355953	11	NULL	NULL	NULL	NULL	Erysipelas	MedicalFinding		is caused by		often			β-hemolytic streptococci	Organism	 group A			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Erysipelas is most often caused by group A (or rarely group C or G) β-hemolytic streptococci and occurs most frequently on the legs and face. However, other causes have been reported, including Staphylococcus aureus (including methicillin-resistant S. aureus [MRSA])	topic_mrs
78674	2	355953	11	NULL	NULL	0	NULL	Erysipelas	MedicalFinding		is caused by		rarely			β-hemolytic streptococci	Organism	group C or G			NULL		0	NULL	NULL	NULL	NULL	NULL	Erysipelas is most often caused by group A (or rarely group C or G) β-hemolytic streptococci and occurs most frequently on the legs and face. However, other causes have been reported, including Staphylococcus aureus (including methicillin-resistant S. aureus [MRSA])	topic_mrs
78675	3	355953	11	NULL	NULL	0	NULL	Erysipelas	MedicalFinding		occurs on		frequently			legs	Organism part				NULL		0	NULL	NULL	NULL	NULL	NULL	Erysipelas is most often caused by group A (or rarely group C or G) β-hemolytic streptococci and occurs most frequently on the legs and face. However, other causes have been reported, including Staphylococcus aureus (including methicillin-resistant S. aureus [MRSA])	topic_mrs
78676	4	355953	11	NULL	NULL	0	NULL	Erysipelas	MedicalFinding		occurs on					face	Organism part				NULL		0	NULL	NULL	NULL	NULL	NULL	Erysipelas is most often caused by group A (or rarely group C or G) β-hemolytic streptococci and occurs most frequently on the legs and face. However, other causes have been reported, including Staphylococcus aureus (including methicillin-resistant S. aureus [MRSA])	topic_mrs
78677	5	355953	11	NULL	NULL	0	NULL	statement 3	Process		occurs along with					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Erysipelas is most often caused by group A (or rarely group C or G) β-hemolytic streptococci and occurs most frequently on the legs and face. However, other causes have been reported, including Staphylococcus aureus (including methicillin-resistant S. aureus [MRSA])	topic_mrs
78678	6	355953	11	NULL	NULL	0	NULL	methicillin-resistant S. aureus	Organism		is					MRSA	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Erysipelas is most often caused by group A (or rarely group C or G) β-hemolytic streptococci and occurs most frequently on the legs and face. However, other causes have been reported, including Staphylococcus aureus (including methicillin-resistant S. aureus [MRSA])	topic_mrs
78679	7	355953	11	NULL	NULL	0	NULL	MRSA	Organism		is a type of 					Staphylococcus aureus	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Erysipelas is most often caused by group A (or rarely group C or G) β-hemolytic streptococci and occurs most frequently on the legs and face. However, other causes have been reported, including Staphylococcus aureus (including methicillin-resistant S. aureus [MRSA])	topic_mrs
78680	8	355953	11	NULL	NULL	0	NULL	MRSA	Organism		causes					Erysipelas	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Erysipelas is most often caused by group A (or rarely group C or G) β-hemolytic streptococci and occurs most frequently on the legs and face. However, other causes have been reported, including Staphylococcus aureus (including methicillin-resistant S. aureus [MRSA])	topic_mrs
76772	1	355954	5	NULL	NULL	0	NULL	Interleukin-1 alpha	GP		is a type of					protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-1 alpha (IL-1α) is a protein	topic_aut
76773	2	355954	5	NULL	NULL	0	NULL	Interleukin-1 alpha	GP		is					IL-1α	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-1 alpha (IL-1α) is a protein	topic_aut
76774	1	355955	5	NULL	NULL	0	NULL	c-Met	GP		is					Mesenchymal??epithelial transition factor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Mesenchymal−epithelial transition factor (c-Met) is a receptor tyrosine kinase	topic_aut
76775	2	355955	5	NULL	NULL	0	NULL	c-Met	GP		is a type of					receptor tyrosine kinase	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Mesenchymal−epithelial transition factor (c-Met) is a receptor tyrosine kinase	topic_aut
76776	1	355956	5	NULL	NULL	0	NULL	MAO	GP		is					Monoamine oxidases	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Monoamine oxidases (MAO) (EC 1.4.3.4) are a family of enzymes	topic_aut
76777	2	355956	5	NULL	NULL	0	NULL	Monoamine oxidases	GP		is a family of					enzymes	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Monoamine oxidases (MAO) (EC 1.4.3.4) are a family of enzymes	topic_aut
76778	1	355957	5	NULL	NULL	0	NULL	proinflammatory cytokine	GP		is a type of					cytokine	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 A proinflammatory cytokine is a cytokine which promotes systemic inflammation	topic_aut
76779	2	355957	5	NULL	NULL	0	NULL	proinflammatory cytokine	GP		promotes					systemic inflammation	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	 A proinflammatory cytokine is a cytokine which promotes systemic inflammation	topic_aut
76780	1	355958	5	NULL	NULL	0	NULL	RTK	GP		is					proto-oncogenic receptor tyrosine kinases	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	proto-oncogenic receptor tyrosine kinases (RTK)s are the high-affinity cell surface receptors 	topic_aut
76781	2	355958	5	NULL	NULL	0	NULL	RTK	GP		is a type of					cell surface receptors	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	proto-oncogenic receptor tyrosine kinases (RTK)s are the high-affinity cell surface receptors 	topic_aut
76782	1	355959	5	NULL	NULL	0	NULL	Sensory integration	Process		is a type of					neurological process	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Sensory integration is defined as the neurological process that organizes sensation from one's own body and the environment	topic_aut
76783	2	355959	5	NULL	NULL	0	NULL	neurological process	Process		organizes					sensation	Process				NULL	body	0	NULL	NULL	NULL	NULL	NULL	Sensory integration is defined as the neurological process that organizes sensation from one's own body and the environment	topic_aut
76784	3	355959	5	NULL	NULL	0	NULL	neurological process	Process		organizes					environment	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	NULL	NULL	Sensory integration is defined as the neurological process that organizes sensation from one's own body and the environment	topic_aut
76785	4	355959	5	NULL	NULL	0	NULL	statement 2	Process		occurs simultaneously with					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Sensory integration is defined as the neurological process that organizes sensation from one's own body and the environment	topic_aut
76786	1	355960	5	NULL	NULL	0	NULL	AD	MedicalFinding		is					autistic disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	patient who was diagnosed with autistic disorder (AD) and responded positively to buspirone, demonstrated by a reduction in target behaviors of self-injury, property destruction, and physical aggression	topic_aut
76787	2	355960	5	NULL	NULL	0	NULL	AD patients	GroupOfPeople		responds to		positively			buspirone	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	patient who was diagnosed with autistic disorder (AD) and responded positively to buspirone, demonstrated by a reduction in target behaviors of self-injury, property destruction, and physical aggression	topic_aut
76788	3	355960	5	NULL	NULL	0	NULL	AD patients	GroupOfPeople		is prone to					self-injury	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	patient who was diagnosed with autistic disorder (AD) and responded positively to buspirone, demonstrated by a reduction in target behaviors of self-injury, property destruction, and physical aggression	topic_aut
76789	4	355960	5	NULL	NULL	0	NULL	AD patients	GroupOfPeople		is prone to					property destruction	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	patient who was diagnosed with autistic disorder (AD) and responded positively to buspirone, demonstrated by a reduction in target behaviors of self-injury, property destruction, and physical aggression	topic_aut
76790	5	355960	5	NULL	NULL	0	NULL	AD patients	GroupOfPeople		is prone to					 physical aggression	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	patient who was diagnosed with autistic disorder (AD) and responded positively to buspirone, demonstrated by a reduction in target behaviors of self-injury, property destruction, and physical aggression	topic_aut
76791	6	355960	5	NULL	NULL	0	NULL	statement 2	Process		reduce					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	patient who was diagnosed with autistic disorder (AD) and responded positively to buspirone, demonstrated by a reduction in target behaviors of self-injury, property destruction, and physical aggression	topic_aut
76792	7	355960	5	NULL	NULL	0	NULL	statement 2	Process		reduce					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	patient who was diagnosed with autistic disorder (AD) and responded positively to buspirone, demonstrated by a reduction in target behaviors of self-injury, property destruction, and physical aggression	topic_aut
76793	8	355960	5	NULL	NULL	0	NULL	statement 2	Process		reduce					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	patient who was diagnosed with autistic disorder (AD) and responded positively to buspirone, demonstrated by a reduction in target behaviors of self-injury, property destruction, and physical aggression	topic_aut
76794	1	355961	5	NULL	NULL	0	NULL	risperidone	Chemical		is a type of					atypical antipsychotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Investigations to date suggest that the atypical antipsychotics such as risperidone have efficacy for certain symptoms of autistic disorder and may be better tolerated than typical antipsychotics	topic_aut
76795	2	355961	5	NULL	NULL	0	NULL	risperidone	Chemical		have efficacy for					autistic disorder	MedicalFinding	certain symptoms of			NULL		0	NULL	NULL	NULL	NULL	NULL	Investigations to date suggest that the atypical antipsychotics such as risperidone have efficacy for certain symptoms of autistic disorder and may be better tolerated than typical antipsychotics	topic_aut
76796	3	355961	5	NULL	NULL	0	NULL	atypical antipsychotics	Chemical		better tolerated than		may be			typical antipsychotics	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Investigations to date suggest that the atypical antipsychotics such as risperidone have efficacy for certain symptoms of autistic disorder and may be better tolerated than typical antipsychotics	topic_aut
76797	1	355962	5	NULL	NULL	0	NULL	haloperidol	Chemical		is a type of					antipsychotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The typical antipsychotic haloperidol is the best-studied medication in autistic disorder but is associated with a high rate of dyskinesias	topic_aut
76798	2	355962	5	NULL	NULL	0	NULL	haloperidol	Chemical		is used to treat					autistic disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The typical antipsychotic haloperidol is the best-studied medication in autistic disorder but is associated with a high rate of dyskinesias	topic_aut
76799	3	355962	5	NULL	NULL	0	NULL	haloperidol	Chemical		is associated with					dyskinesias	MedicalFinding	high rate of			NULL		0	NULL	NULL	NULL	NULL	NULL	The typical antipsychotic haloperidol is the best-studied medication in autistic disorder but is associated with a high rate of dyskinesias	topic_aut
76800	1	355963	5	NULL	NULL	0	NULL	Dyskinesia	MedicalFinding		is a type of					movement disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Dyskinesia is a movement disorder which consists of effects including diminished voluntary movements[1] and the presence of involuntary movements, similar to tics or chorea	topic_aut
76801	2	355963	5	NULL	NULL	0	NULL	voluntary movements	PhysicalPhenomenon		is diminished in					Dyskinesia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Dyskinesia is a movement disorder which consists of effects including diminished voluntary movements[1] and the presence of involuntary movements, similar to tics or chorea	topic_aut
76802	3	355963	5	NULL	NULL	0	NULL	involuntary movements	PhysicalPhenomenon		is present in					Dyskinesia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Dyskinesia is a movement disorder which consists of effects including diminished voluntary movements[1] and the presence of involuntary movements, similar to tics or chorea	topic_aut
76803	4	355963	5	NULL	NULL	0	NULL	tics	MedicalFinding		is a type of					involuntary movement	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	NULL	NULL	Dyskinesia is a movement disorder which consists of effects including diminished voluntary movements[1] and the presence of involuntary movements, similar to tics or chorea	topic_aut
76804	5	355963	5	NULL	NULL	0	NULL	chorea	MedicalFinding		is a type of					involuntary movement	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	NULL	NULL	Dyskinesia is a movement disorder which consists of effects including diminished voluntary movements[1] and the presence of involuntary movements, similar to tics or chorea	topic_aut
76805	1	355964	5	NULL	NULL	NULL	NULL	hyperactivity	MedicalFinding		is observed in					autistic children	GroupOfPeople				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Psychostimulants reduced hyperactivity and irritability in one small double-blind crossover study in children with autistic disorder, although these agents are frequently reported to exacerbate irritability, insomnia, and aggression in clinical populations	topic_aut
76806	2	355964	5	NULL	NULL	0	NULL	irritability	MedicalFinding		is observed in					autistic children	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Psychostimulants reduced hyperactivity and irritability in one small double-blind crossover study in children with autistic disorder, although these agents are frequently reported to exacerbate irritability, insomnia, and aggression in clinical populations	topic_aut
76807	3	355964	5	NULL	NULL	0	NULL	Psychostimulants	Chemical		reduce					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Psychostimulants reduced hyperactivity and irritability in one small double-blind crossover study in children with autistic disorder, although these agents are frequently reported to exacerbate irritability, insomnia, and aggression in clinical populations	topic_aut
76808	4	355964	5	NULL	NULL	0	NULL	Psychostimulants	Chemical		reduce					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Psychostimulants reduced hyperactivity and irritability in one small double-blind crossover study in children with autistic disorder, although these agents are frequently reported to exacerbate irritability, insomnia, and aggression in clinical populations	topic_aut
76809	5	355964	5	NULL	NULL	0	NULL	Psychostimulants	Chemical		exacerbate					irritability	MedicalFinding				NULL	clinical populations	0	NULL	NULL	NULL	NULL	NULL	Psychostimulants reduced hyperactivity and irritability in one small double-blind crossover study in children with autistic disorder, although these agents are frequently reported to exacerbate irritability, insomnia, and aggression in clinical populations	topic_aut
76810	6	355964	5	NULL	NULL	0	NULL	Psychostimulants	Chemical		exacerbate					insomnia	MedicalFinding				NULL	clinical populations	0	NULL	NULL	NULL	NULL	NULL	Psychostimulants reduced hyperactivity and irritability in one small double-blind crossover study in children with autistic disorder, although these agents are frequently reported to exacerbate irritability, insomnia, and aggression in clinical populations	topic_aut
76811	7	355964	5	NULL	NULL	0	NULL	Psychostimulants	Chemical		exacerbate					aggression	MedicalFinding				NULL	clinical populations	0	NULL	NULL	NULL	NULL	NULL	Psychostimulants reduced hyperactivity and irritability in one small double-blind crossover study in children with autistic disorder, although these agents are frequently reported to exacerbate irritability, insomnia, and aggression in clinical populations	topic_aut
76812	1	355965	5	NULL	NULL	NULL	NULL	sertraline	Chemical	small doses of	is effective in		may be			anxiety	MedicalFinding	treatment of;;symptoms of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our experience suggests that small doses of sertraline may be effective for treating symptoms of anxiety and agitation	topic_aut
76813	2	355965	5	NULL	NULL	NULL	NULL	sertraline	Chemical	small doses of	is effective in		may be			agitation	MedicalFinding	treatment of;;symptoms of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our experience suggests that small doses of sertraline may be effective for treating symptoms of anxiety and agitation	topic_aut
76814	1	355966	5	NULL	NULL	NULL	NULL	Sertraline hydrochloride	Chemical		is a type of					generic antidepressant	Chemical				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Sertraline hydrochloride (trade names Zoloft and Lustral) is a generic antidepressant	topic_aut
76815	2	355966	5	NULL	NULL	0	NULL	Zoloft	Chemical		is the trade name of					Sertraline hydrochloride	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Sertraline hydrochloride (trade names Zoloft and Lustral) is a generic antidepressant	topic_aut
76816	3	355966	5	NULL	NULL	0	NULL	Lustral	Chemical		is the trade name of					Sertraline hydrochloride	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Sertraline hydrochloride (trade names Zoloft and Lustral) is a generic antidepressant	topic_aut
76817	1	355967	5	NULL	NULL	0	NULL	irritability	MedicalFinding	high rate of	is observed in					autistic children	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Children with autism and autism spectrum disorders have a high rate of irritability and aggressive symptoms	topic_aut
76818	2	355967	5	NULL	NULL	0	NULL	irritability	MedicalFinding	high rate of	is observed in					autism spectrum disorder children	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Children with autism and autism spectrum disorders have a high rate of irritability and aggressive symptoms	topic_aut
76819	3	355967	5	NULL	NULL	0	NULL	aggressive symptoms	MedicalFinding	high rate of	is observed in					autistic children	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Children with autism and autism spectrum disorders have a high rate of irritability and aggressive symptoms	topic_aut
76820	4	355967	5	NULL	NULL	NULL	NULL	aggressive symptoms	MedicalFinding	high rate of	is observed in					autism spectrum disorder children	GroupOfPeople				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Children with autism and autism spectrum disorders have a high rate of irritability and aggressive symptoms	topic_aut
76821	1	355968	5	NULL	NULL	0	NULL	irritability	MedicalFinding		is a symptom of					autistic children	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	children with autism have symptoms of irritability and aggression including aggression, severe tantrums, and deliberate self injurious behavior	topic_aut
76822	2	355968	5	NULL	NULL	0	NULL	aggression	MedicalFinding		is a symptom of					autistic children	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	children with autism have symptoms of irritability and aggression including aggression, severe tantrums, and deliberate self injurious behavior	topic_aut
76823	3	355968	5	NULL	NULL	0	NULL	tantrums	MedicalFinding	severe	is a symptom of					autistic children	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	children with autism have symptoms of irritability and aggression including aggression, severe tantrums, and deliberate self injurious behavior	topic_aut
76824	4	355968	5	NULL	NULL	0	NULL	self injurious behavior	MedicalFinding	delibrate	is a symptom of					autistic children	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	children with autism have symptoms of irritability and aggression including aggression, severe tantrums, and deliberate self injurious behavior	topic_aut
76825	1	355969	5	NULL	NULL	0	NULL	Aripiprazole	Chemical		is a type of					atypical antipsychotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Aripiprazole is an atypical or newer generation antipsychotic with a unique mechanism of action impacting dopaminergic and serotonergic neurotransmission. The drug has been found efficacious for several indications, including most recently for use targeting irritability associated with autistic disorder	topic_aut
76826	2	355969	5	NULL	NULL	0	NULL	Aripiprazole	Chemical		is a type of					newer generation antipsychotic	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Aripiprazole is an atypical or newer generation antipsychotic with a unique mechanism of action impacting dopaminergic and serotonergic neurotransmission. The drug has been found efficacious for several indications, including most recently for use targeting irritability associated with autistic disorder	topic_aut
76827	3	355969	5	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Aripiprazole is an atypical or newer generation antipsychotic with a unique mechanism of action impacting dopaminergic and serotonergic neurotransmission. The drug has been found efficacious for several indications, including most recently for use targeting irritability associated with autistic disorder	topic_aut
76828	4	355969	5	NULL	NULL	0	NULL	Aripiprazole	Chemical		impact					dopaminergic neurotransmission	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Aripiprazole is an atypical or newer generation antipsychotic with a unique mechanism of action impacting dopaminergic and serotonergic neurotransmission. The drug has been found efficacious for several indications, including most recently for use targeting irritability associated with autistic disorder	topic_aut
76829	5	355969	5	NULL	NULL	0	NULL	Aripiprazole	Chemical		impact					serotonergic neurotransmission	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Aripiprazole is an atypical or newer generation antipsychotic with a unique mechanism of action impacting dopaminergic and serotonergic neurotransmission. The drug has been found efficacious for several indications, including most recently for use targeting irritability associated with autistic disorder	topic_aut
76830	6	355969	5	NULL	NULL	0	NULL	irritability	MedicalFinding		is associated with					autistic disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Aripiprazole is an atypical or newer generation antipsychotic with a unique mechanism of action impacting dopaminergic and serotonergic neurotransmission. The drug has been found efficacious for several indications, including most recently for use targeting irritability associated with autistic disorder	topic_aut
76831	7	355969	5	NULL	NULL	0	NULL	Aripiprazole	Chemical		is efficacious for					statement 6	Process	targeting			NULL		0	NULL	NULL	NULL	NULL	NULL	Aripiprazole is an atypical or newer generation antipsychotic with a unique mechanism of action impacting dopaminergic and serotonergic neurotransmission. The drug has been found efficacious for several indications, including most recently for use targeting irritability associated with autistic disorder	topic_aut
77390	1	355970	7	NULL	NULL	0	NULL	PKCβ1 isoform	GP		expressed in					B-ALL cell line	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of PKCβ1 and PKCβ2 isoforms was demonstrated in five B-ALL cell lines characterized by distinctive chromosomal translocations	topic_ll
77391	2	355970	7	NULL	NULL	0	NULL	PKCβ2 isoform	GP		expressed in					B-ALL cell line	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of PKCβ1 and PKCβ2 isoforms was demonstrated in five B-ALL cell lines characterized by distinctive chromosomal translocations	topic_ll
77394	1	355972	7	NULL	NULL	NULL	NULL	B-ALL cell lines	Cell		express					PKCβ1 isoform	GP				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Expression of PKCβ1 and PKCβ2 isoforms was demonstrated in five B-ALL cell lines characterized by distinctive chromosomal translocations, and sensitivity to PKCβ-selective inhibition was examined. Inhibitor treatment resulted in a dose-dependent reduction in viability in all cell lines, although pro-B ALL with t(4;11)(q21;q23) was most sensitive.	topic_ll
77395	2	355972	7	NULL	NULL	0	NULL	B-ALL cell lines	Cell		express					PKCβ2 isoform	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of PKCβ1 and PKCβ2 isoforms was demonstrated in five B-ALL cell lines characterized by distinctive chromosomal translocations, and sensitivity to PKCβ-selective inhibition was examined. Inhibitor treatment resulted in a dose-dependent reduction in viability in all cell lines, although pro-B ALL with t(4;11)(q21;q23) was most sensitive.	topic_ll
77396	3	355972	7	NULL	NULL	NULL	NULL	Inhibitor	Chemical	treatment 	reduce		dose-dependently			viability	Process				NULL	cell lines	NULL	NULL	NULL	NULL	NULL	NULL	Expression of PKCβ1 and PKCβ2 isoforms was demonstrated in five B-ALL cell lines characterized by distinctive chromosomal translocations, and sensitivity to PKCβ-selective inhibition was examined. Inhibitor treatment resulted in a dose-dependent reduction in viability in all cell lines, although pro-B ALL with t(4;11)(q21;q23) was most sensitive.	topic_ll
77397	4	355972	7	NULL	NULL	0	NULL	 pro-B ALL	MedicalFinding		contains									t(4;11)(q21;q23)	NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of PKCβ1 and PKCβ2 isoforms was demonstrated in five B-ALL cell lines characterized by distinctive chromosomal translocations, and sensitivity to PKCβ-selective inhibition was examined. Inhibitor treatment resulted in a dose-dependent reduction in viability in all cell lines, although pro-B ALL with t(4;11)(q21;q23) was most sensitive.	topic_ll
77398	5	355972	7	NULL	NULL	0	NULL	 pro-B ALL 	MedicalFinding		is sensitive to					inhibitor	Chemical	treatment with			NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of PKCβ1 and PKCβ2 isoforms was demonstrated in five B-ALL cell lines characterized by distinctive chromosomal translocations, and sensitivity to PKCβ-selective inhibition was examined. Inhibitor treatment resulted in a dose-dependent reduction in viability in all cell lines, although pro-B ALL with t(4;11)(q21;q23) was most sensitive.	topic_ll
77399	1	355973	7	NULL	NULL	0	NULL	PKCβ	GP	targeting	treatment for					B-ALL	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that PKCβ targeting should be considered as a potential treatment option in B-ALL. NULL	topic_ll
77400	1	355975	7	NULL	NULL	0	NULL	oxidative stress	Process	increased	occur in					acute lymphoblastic leukemia	MedicalFinding	childhood			NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of anti-oxidant status and apoptosis on the induction phase of chemotherapy in childhood acute lymphoblastic leukemia.Our study showed that there was increased oxidative stress at diagnosis and after treatment with chemotherapy. 	topic_ll
77401	2	355975	7	NULL	NULL	0	NULL	statement 1	Process		occur during					diagnosis	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of anti-oxidant status and apoptosis on the induction phase of chemotherapy in childhood acute lymphoblastic leukemia.Our study showed that there was increased oxidative stress at diagnosis and after treatment with chemotherapy. 	topic_ll
77402	3	355975	7	NULL	NULL	0	NULL	statement 1	Process		occur after					chemotherapy	MedicalProcedure	treatment with			NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of anti-oxidant status and apoptosis on the induction phase of chemotherapy in childhood acute lymphoblastic leukemia.Our study showed that there was increased oxidative stress at diagnosis and after treatment with chemotherapy. 	topic_ll
77403	4	355975	7	NULL	NULL	0	NULL	statement 2	Process		occur along with					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of anti-oxidant status and apoptosis on the induction phase of chemotherapy in childhood acute lymphoblastic leukemia.Our study showed that there was increased oxidative stress at diagnosis and after treatment with chemotherapy. 	topic_ll
78053	1	355976	6	NULL	NULL	0	NULL	Mucinous carcinomas	MedicalFinding		accounts for					Breast cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mucinous carcinomas are a rare entity accounting for up to 2% of all breast cancers, which have been shown to display a gene expression profile distinct from that of invasive ductal carcinomas of no special type (IDC-NSTs)	topic_bc
78054	1	355977	6	NULL	NULL	0	NULL	PTEN gene	GP	mutation of	is found in					breast carcinoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of heterozygosity (LOH) in loci of the 10q23 region that harbor the PTEN gene and mutations in the sequence of this gene have been found in several primary human tumors including breast carcinomas	topic_bc
78055	2	355977	6	NULL	NULL	0	NULL	PTEN	GP		is located on					chromosome 10q23					NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of heterozygosity (LOH) in loci of the 10q23 region that harbor the PTEN gene and mutations in the sequence of this gene have been found in several primary human tumors including breast carcinomas	topic_bc
78056	1	355978	6	NULL	NULL	0	NULL	CDK inhibitors	Chemical		serve as					Breast cancer	MedicalFinding	therapeutics for			NULL		0	NULL	NULL	NULL	NULL	NULL	CDK inhibitors as potential breast cancer therapeutics: new evidence for enhanced efficacy in ER+ disease	topic_bc
78057	1	355979	6	NULL	NULL	0	NULL	CDK inhibitor	Chemical		inhibits					CDK	GP	function of 			NULL		0	NULL	NULL	NULL	NULL	NULL	A CDK (Cyclin-dependent kinase) inhibitor is a chemical that inhibits the function of CDKs	topic_bc
78058	2	355979	6	NULL	NULL	0	NULL	CDK	GP		is					Cyclin-dependent kinase	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	A CDK (Cyclin-dependent kinase) inhibitor is a chemical that inhibits the function of CDKs	topic_bc
77404	1	355980	7	NULL	NULL	NULL	NULL	BD	MedicalFinding		associated with					neurocognitive deficits	MedicalFinding	significant			NULL		NULL	NULL	NULL	NULL	NULL	NULL	There is evidence that bipolar disorder (BD) is associated with significant neurocognitive deficits and this occurs in individuals with BD type I (BD I) and with BD type II (BD II). 	topic_bd
77405	2	355980	7	NULL	NULL	NULL	NULL	neurocognitive deficits	MedicalFinding	significant	occur in					BD I	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	There is evidence that bipolar disorder (BD) is associated with significant neurocognitive deficits and this occurs in individuals with BD type I (BD I) and with BD type II (BD II). 	topic_bd
77406	3	355980	7	NULL	NULL	NULL	NULL	neurocognitive deficits	MedicalFinding	significant	occur in					BD II	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	There is evidence that bipolar disorder (BD) is associated with significant neurocognitive deficits and this occurs in individuals with BD type I (BD I) and with BD type II (BD II). 	topic_bd
77407	4	355980	7	NULL	NULL	NULL	NULL	BD	MedicalFinding		is					bipolar disorder	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	There is evidence that bipolar disorder (BD) is associated with significant neurocognitive deficits and this occurs in individuals with BD type I (BD I) and with BD type II (BD II). 	topic_bd
77408	5	355980	7	NULL	NULL	0	NULL	BD I	MedicalFinding		is					BD type I	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	There is evidence that bipolar disorder (BD) is associated with significant neurocognitive deficits and this occurs in individuals with BD type I (BD I) and with BD type II (BD II). 	topic_bd
77409	6	355980	7	NULL	NULL	0	NULL	BD II	MedicalFinding		is					BD type II	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	There is evidence that bipolar disorder (BD) is associated with significant neurocognitive deficits and this occurs in individuals with BD type I (BD I) and with BD type II (BD II). 	topic_bd
77410	1	355981	7	NULL	NULL	0	NULL	Main cognitive deficits	MedicalFinding		observed in					BD II	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Main cognitive deficits found in BD II include working memory and some measures of executive functions (inhibitory control) and approximately half of the studies also detected verbal memory impairment.	topic_bd
77411	2	355981	7	NULL	NULL	0	NULL	statement 1	Process		include					working memory	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Main cognitive deficits found in BD II include working memory and some measures of executive functions (inhibitory control) and approximately half of the studies also detected verbal memory impairment.	topic_bd
77412	3	355981	7	NULL	NULL	0	NULL	statement 1	Process		include					verbal memory impairment	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Main cognitive deficits found in BD II include working memory and some measures of executive functions (inhibitory control) and approximately half of the studies also detected verbal memory impairment.	topic_bd
76832	1	355982	5	NULL	NULL	0	NULL	CNTNAP2 protein	GP		is active in					brain	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	CNTNAP2 encodes a protein active in the brain during development. One particular variant in the gene was first linked to autism in 2006. Later studies have also implicated CNTNAP2 variants in specific language impairment, ADHD, Tourette syndrome, and schizophrenia.	topic_aut
76833	2	355982	5	NULL	NULL	0	NULL	statement 1	Process		occurs during					development	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	CNTNAP2 encodes a protein active in the brain during development. One particular variant in the gene was first linked to autism in 2006. Later studies have also implicated CNTNAP2 variants in specific language impairment, ADHD, Tourette syndrome, and schizophrenia.	topic_aut
76834	3	355982	5	NULL	NULL	0	NULL	CNTNAP2 variant	GP		is linked to					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	CNTNAP2 encodes a protein active in the brain during development. One particular variant in the gene was first linked to autism in 2006. Later studies have also implicated CNTNAP2 variants in specific language impairment, ADHD, Tourette syndrome, and schizophrenia.	topic_aut
76835	4	355982	5	NULL	NULL	NULL	NULL	CNTNAP2 variant	GP		is implicated in					language impairment	MedicalFinding	specific			NULL		NULL	NULL	NULL	NULL	NULL	NULL	CNTNAP2 encodes a protein active in the brain during development. One particular variant in the gene was first linked to autism in 2006. Later studies have also implicated CNTNAP2 variants in specific language impairment, ADHD, Tourette syndrome, and schizophrenia.	topic_aut
76836	5	355982	5	NULL	NULL	0	NULL	CNTNAP2 variant	GP		is implicated in					ADHD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	CNTNAP2 encodes a protein active in the brain during development. One particular variant in the gene was first linked to autism in 2006. Later studies have also implicated CNTNAP2 variants in specific language impairment, ADHD, Tourette syndrome, and schizophrenia.	topic_aut
76837	6	355982	5	NULL	NULL	0	NULL	CNTNAP2 variant	GP		is implicated in					Tourette syndrome	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	CNTNAP2 encodes a protein active in the brain during development. One particular variant in the gene was first linked to autism in 2006. Later studies have also implicated CNTNAP2 variants in specific language impairment, ADHD, Tourette syndrome, and schizophrenia.	topic_aut
76838	7	355982	5	NULL	NULL	0	NULL	CNTNAP2 variant	GP		is implicated in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	CNTNAP2 encodes a protein active in the brain during development. One particular variant in the gene was first linked to autism in 2006. Later studies have also implicated CNTNAP2 variants in specific language impairment, ADHD, Tourette syndrome, and schizophrenia.	topic_aut
76839	1	355983	5	NULL	NULL	0	NULL	neuroligin-3 protein	GP		is involved in					autism	MedicalFinding	gene mutation of			NULL		0	NULL	NULL	NULL	NULL	NULL	At U.C. San Diego, lead researcher Dr. Palmer Taylor says autism’s gene mutation involves a protein called neuroligin-3, which appears to prevent normal communication between the nerves.	topic_aut
76840	2	355983	5	NULL	NULL	NULL	NULL	communication	Process	normal	is present between					nerves	OrganismPart				NULL		NULL	NULL	NULL	NULL	NULL	NULL	At U.C. San Diego, lead researcher Dr. Palmer Taylor says autism’s gene mutation involves a protein called neuroligin-3, which appears to prevent normal communication between the nerves.	topic_aut
76841	3	355983	5	NULL	NULL	0	NULL	neuroligin-3 protein	GP		prevent					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	At U.C. San Diego, lead researcher Dr. Palmer Taylor says autism’s gene mutation involves a protein called neuroligin-3, which appears to prevent normal communication between the nerves.	topic_aut
76842	1	355984	5	NULL	NULL	0	NULL	PTCHD1 gene	GP		is present in					X chromosome	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	The research data found that 1% of boys affected with ASD had mutations that are linked with the PTCHD1 gene on the X chromosome.	topic_aut
76843	2	355984	5	NULL	NULL	0	NULL	PTCHD1 gene	GP	mutation of	is linked to					ASD	MedicalFinding				NULL	boys	0	NULL	NULL	NULL	NULL	NULL	The research data found that 1% of boys affected with ASD had mutations that are linked with the PTCHD1 gene on the X chromosome.	topic_aut
77413	1	355985	7	NULL	NULL	0	NULL	 hypovitaminosis D	MedicalFinding		associated with					basic cognitive functions	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Several studies suggest an association between hypovitaminosis D and basic and executive cognitive functions, depression, bipolar disorder, and schizophrenia.	topic_bd
77414	2	355985	7	NULL	NULL	0	NULL	hypovitaminosis D	MedicalFinding		associated with					executive cognitive functions	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Several studies suggest an association between hypovitaminosis D and basic and executive cognitive functions, depression, bipolar disorder, and schizophrenia.	topic_bd
77415	3	355985	7	NULL	NULL	0	NULL	hypovitaminosis D	MedicalFinding		associated with					depression	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Several studies suggest an association between hypovitaminosis D and basic and executive cognitive functions, depression, bipolar disorder, and schizophrenia.	topic_bd
77416	4	355985	7	NULL	NULL	0	NULL	hypovitaminosis D	MedicalFinding		associated with					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Several studies suggest an association between hypovitaminosis D and basic and executive cognitive functions, depression, bipolar disorder, and schizophrenia.	topic_bd
77417	5	355985	7	NULL	NULL	0	NULL	hypovitaminosis D	MedicalFinding		associated with					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Several studies suggest an association between hypovitaminosis D and basic and executive cognitive functions, depression, bipolar disorder, and schizophrenia.	topic_bd
76844	1	355986	5	NULL	NULL	0	NULL	gene	GP	certain versions of	is present in					chromosome 7	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	In the inherited form of risk, people with autism were more prone than healthy controls to have certain versions of a gene on Chromosome 7	topic_aut
76845	2	355986	5	NULL	NULL	NULL	NULL	healthy control	Organism		contains					statement 1	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the inherited form of risk, people with autism were more prone than healthy controls to have certain versions of a gene on Chromosome 7	topic_aut
76846	3	355986	5	NULL	NULL	NULL	NULL	autistic people	GroupOfPeople		contains					statement 1	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the inherited form of risk, people with autism were more prone than healthy controls to have certain versions of a gene on Chromosome 7	topic_aut
76847	4	355986	5	NULL	NULL	0	NULL	statement 3	Process		more prone than					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	In the inherited form of risk, people with autism were more prone than healthy controls to have certain versions of a gene on Chromosome 7	topic_aut
76848	1	355987	5	NULL	NULL	0	NULL	gene	GP		is missing on					chromosome 16	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	In the spontaneous form, one percent of autism was traced to a conspicuous 'hot spot' of missing or duplicated genes on Chromosome 16.	topic_aut
76849	2	355987	5	NULL	NULL	0	NULL	gene	GP		is duplicated on					chromosome 16	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	In the spontaneous form, one percent of autism was traced to a conspicuous 'hot spot' of missing or duplicated genes on Chromosome 16.	topic_aut
76850	3	355987	5	NULL	NULL	0	NULL	autism	MedicalFinding	one percent of	is traced to					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	In the spontaneous form, one percent of autism was traced to a conspicuous 'hot spot' of missing or duplicated genes on Chromosome 16.	topic_aut
76851	4	355987	5	NULL	NULL	0	NULL	autism	MedicalFinding	one percent of	is traced to					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	In the spontaneous form, one percent of autism was traced to a conspicuous 'hot spot' of missing or duplicated genes on Chromosome 16.	topic_aut
76852	5	355987	5	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	In the spontaneous form, one percent of autism was traced to a conspicuous 'hot spot' of missing or duplicated genes on Chromosome 16.	topic_aut
76853	1	355989	5	NULL	NULL	0	NULL	CNTNAP2	GP		is present in					chromosome 7	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	Also drawing upon the AGRE resource, three other teams of researchers independently linked inherited variation in a gene on Chromosome 7, called CNTNAP2, with autism. 	topic_aut
76854	2	355989	5	NULL	NULL	0	NULL	CNTNAP2	GP		is linked to					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Also drawing upon the AGRE resource, three other teams of researchers independently linked inherited variation in a gene on Chromosome 7, called CNTNAP2, with autism. 	topic_aut
77418	1	355990	7	NULL	NULL	0	NULL	Ion dysregulation	Process		involved in		may be			bipolar illness	MedicalFinding	pathophysiology of			NULL		0	NULL	NULL	NULL	NULL	NULL	Ion dysregulation is thought to be involved in the pathophysiology of bipolar illness, suggesting that memantine may be effective in treating bipolar manic and/or depressive episodes. 	topic_bd
77419	2	355990	7	NULL	NULL	0	NULL	memantine	Chemical		effective in		may be			bipolar manic episode	MedicalFinding	treating			NULL		0	NULL	NULL	NULL	NULL	NULL	Ion dysregulation is thought to be involved in the pathophysiology of bipolar illness, suggesting that memantine may be effective in treating bipolar manic and/or depressive episodes. 	topic_bd
77420	3	355990	7	NULL	NULL	0	NULL	memantine	Chemical		effective in		may be			bipolar depressive episodes	MedicalFinding	treating			NULL		0	NULL	NULL	NULL	NULL	NULL	Ion dysregulation is thought to be involved in the pathophysiology of bipolar illness, suggesting that memantine may be effective in treating bipolar manic and/or depressive episodes. 	topic_bd
77421	4	355990	7	NULL	NULL	0	NULL	statement 1	Process		suggest					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Ion dysregulation is thought to be involved in the pathophysiology of bipolar illness, suggesting that memantine may be effective in treating bipolar manic and/or depressive episodes. 	topic_bd
77422	5	355990	7	NULL	NULL	0	NULL	statement 1	Process		suggest					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Ion dysregulation is thought to be involved in the pathophysiology of bipolar illness, suggesting that memantine may be effective in treating bipolar manic and/or depressive episodes. 	topic_bd
76855	1	355991	5	NULL	NULL	0	NULL	NCAM2	GP		is					neural cell adhesion molecule 2	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	One of the new genes identified was neural cell adhesion molecule 2 (NCAM2). NCAM2 is expressed in the hippocampus of the human brain -- a region previously associated with autism.	topic_aut
76856	3	355991	5	NULL	NULL	NULL	NULL	NCAM2	GP		expressed in					statement 2	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	One of the new genes identified was neural cell adhesion molecule 2 (NCAM2). NCAM2 is expressed in the hippocampus of the human brain -- a region previously associated with autism.	topic_aut
76857	2	355991	5	NULL	NULL	0	NULL	hippocampus	OrganismPart	human	is present in					brain	OrganismPart	human			NULL		0	NULL	NULL	NULL	NULL	NULL	One of the new genes identified was neural cell adhesion molecule 2 (NCAM2). NCAM2 is expressed in the hippocampus of the human brain -- a region previously associated with autism.	topic_aut
76858	4	355991	5	NULL	NULL	0	NULL	statement 2	Process		is associated with		previously			autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	One of the new genes identified was neural cell adhesion molecule 2 (NCAM2). NCAM2 is expressed in the hippocampus of the human brain -- a region previously associated with autism.	topic_aut
77423	1	355992	7	NULL	NULL	0	NULL	 hippocampal slices	OrganismPart	rat	treated with					ouabain 	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	In a second model of bipolar disorder, cycling between population spikes and epileptiform bursts was investigated in rat hippocampal slices treated with ouabain (3.3μM) alone or in combination with memantine (0.5, 1.0, and 5.0μM). Ouabain-induced hyperlocomotion was normalized with acute and chronic lithium and chronic use of memantine. Memantine delayed the onset of ouabain-induced-cycling in hippocampal slices. Memantine may have antimanic properties.	topic_bd
77424	2	355992	7	NULL	NULL	0	NULL	population spikes 	MedicalFinding		cycle between					epileptiform bursts	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In a second model of bipolar disorder, cycling between population spikes and epileptiform bursts was investigated in rat hippocampal slices treated with ouabain (3.3μM) alone or in combination with memantine (0.5, 1.0, and 5.0μM). Ouabain-induced hyperlocomotion was normalized with acute and chronic lithium and chronic use of memantine. Memantine delayed the onset of ouabain-induced-cycling in hippocampal slices. Memantine may have antimanic properties.	topic_bd
77425	3	355992	7	NULL	NULL	0	NULL	statement 2	Process		occur upon					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	In a second model of bipolar disorder, cycling between population spikes and epileptiform bursts was investigated in rat hippocampal slices treated with ouabain (3.3μM) alone or in combination with memantine (0.5, 1.0, and 5.0μM). Ouabain-induced hyperlocomotion was normalized with acute and chronic lithium and chronic use of memantine. Memantine delayed the onset of ouabain-induced-cycling in hippocampal slices. Memantine may have antimanic properties.	topic_bd
77426	4	355992	7	NULL	NULL	0	NULL	statement 1	Process		treated with					memantine 	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	In a second model of bipolar disorder, cycling between population spikes and epileptiform bursts was investigated in rat hippocampal slices treated with ouabain (3.3μM) alone or in combination with memantine (0.5, 1.0, and 5.0μM). Ouabain-induced hyperlocomotion was normalized with acute and chronic lithium and chronic use of memantine. Memantine delayed the onset of ouabain-induced-cycling in hippocampal slices. Memantine may have antimanic properties.	topic_bd
77427	5	355992	7	NULL	NULL	0	NULL	statement 2	Process		occur upon					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	In a second model of bipolar disorder, cycling between population spikes and epileptiform bursts was investigated in rat hippocampal slices treated with ouabain (3.3μM) alone or in combination with memantine (0.5, 1.0, and 5.0μM). Ouabain-induced hyperlocomotion was normalized with acute and chronic lithium and chronic use of memantine. Memantine delayed the onset of ouabain-induced-cycling in hippocampal slices. Memantine may have antimanic properties.	topic_bd
77428	6	355992	7	NULL	NULL	0	NULL	statement 3	Process		is an alternative to					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	In a second model of bipolar disorder, cycling between population spikes and epileptiform bursts was investigated in rat hippocampal slices treated with ouabain (3.3μM) alone or in combination with memantine (0.5, 1.0, and 5.0μM). Ouabain-induced hyperlocomotion was normalized with acute and chronic lithium and chronic use of memantine. Memantine delayed the onset of ouabain-induced-cycling in hippocampal slices. Memantine may have antimanic properties.	topic_bd
77429	7	355992	7	NULL	NULL	0	NULL	Ouabain	GP		induce					hyperlocomotion	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	In a second model of bipolar disorder, cycling between population spikes and epileptiform bursts was investigated in rat hippocampal slices treated with ouabain (3.3μM) alone or in combination with memantine (0.5, 1.0, and 5.0μM). Ouabain-induced hyperlocomotion was normalized with acute and chronic lithium and chronic use of memantine. Memantine delayed the onset of ouabain-induced-cycling in hippocampal slices. Memantine may have antimanic properties.	topic_bd
77430	8	355992	7	NULL	NULL	0	NULL	statement 7	Process		normalized with					acute lithium	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	In a second model of bipolar disorder, cycling between population spikes and epileptiform bursts was investigated in rat hippocampal slices treated with ouabain (3.3μM) alone or in combination with memantine (0.5, 1.0, and 5.0μM). Ouabain-induced hyperlocomotion was normalized with acute and chronic lithium and chronic use of memantine. Memantine delayed the onset of ouabain-induced-cycling in hippocampal slices. Memantine may have antimanic properties.	topic_bd
77431	9	355992	7	NULL	NULL	0	NULL	statement 7	Process		normalized with					chronic lithium	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	In a second model of bipolar disorder, cycling between population spikes and epileptiform bursts was investigated in rat hippocampal slices treated with ouabain (3.3μM) alone or in combination with memantine (0.5, 1.0, and 5.0μM). Ouabain-induced hyperlocomotion was normalized with acute and chronic lithium and chronic use of memantine. Memantine delayed the onset of ouabain-induced-cycling in hippocampal slices. Memantine may have antimanic properties.	topic_bd
77432	10	355992	7	NULL	NULL	0	NULL	statement 7	Process		normalized with					memantine 	Chemical	chronic use of			NULL		0	NULL	NULL	NULL	NULL	NULL	In a second model of bipolar disorder, cycling between population spikes and epileptiform bursts was investigated in rat hippocampal slices treated with ouabain (3.3μM) alone or in combination with memantine (0.5, 1.0, and 5.0μM). Ouabain-induced hyperlocomotion was normalized with acute and chronic lithium and chronic use of memantine. Memantine delayed the onset of ouabain-induced-cycling in hippocampal slices. Memantine may have antimanic properties.	topic_bd
77433	11	355992	7	NULL	NULL	0	NULL	ouabain	GP		induce					cycling	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	In a second model of bipolar disorder, cycling between population spikes and epileptiform bursts was investigated in rat hippocampal slices treated with ouabain (3.3μM) alone or in combination with memantine (0.5, 1.0, and 5.0μM). Ouabain-induced hyperlocomotion was normalized with acute and chronic lithium and chronic use of memantine. Memantine delayed the onset of ouabain-induced-cycling in hippocampal slices. Memantine may have antimanic properties.	topic_bd
77434	12	355992	7	NULL	NULL	0	NULL	statement 11	Process		occur in					hippocampal slices	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	In a second model of bipolar disorder, cycling between population spikes and epileptiform bursts was investigated in rat hippocampal slices treated with ouabain (3.3μM) alone or in combination with memantine (0.5, 1.0, and 5.0μM). Ouabain-induced hyperlocomotion was normalized with acute and chronic lithium and chronic use of memantine. Memantine delayed the onset of ouabain-induced-cycling in hippocampal slices. Memantine may have antimanic properties.	topic_bd
77435	13	355992	7	NULL	NULL	0	NULL	Memantine 	Chemical		delays					statement 11	Process	onset of			NULL		0	NULL	NULL	NULL	NULL	NULL	In a second model of bipolar disorder, cycling between population spikes and epileptiform bursts was investigated in rat hippocampal slices treated with ouabain (3.3μM) alone or in combination with memantine (0.5, 1.0, and 5.0μM). Ouabain-induced hyperlocomotion was normalized with acute and chronic lithium and chronic use of memantine. Memantine delayed the onset of ouabain-induced-cycling in hippocampal slices. Memantine may have antimanic properties.	topic_bd
77436	14	355992	7	NULL	NULL	0	NULL	Memantine	Chemical		have		may			antimanic properties	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In a second model of bipolar disorder, cycling between population spikes and epileptiform bursts was investigated in rat hippocampal slices treated with ouabain (3.3μM) alone or in combination with memantine (0.5, 1.0, and 5.0μM). Ouabain-induced hyperlocomotion was normalized with acute and chronic lithium and chronic use of memantine. Memantine delayed the onset of ouabain-induced-cycling in hippocampal slices. Memantine may have antimanic properties.	topic_bd
77437	1	355993	7	NULL	NULL	0	NULL	cannabis 	Organism	excessive	associated with					bipolar disorder	MedicalFinding	earlier age at onset			NULL		0	NULL	NULL	NULL	NULL	NULL	Excessive cannabis use is associated with earlier age at onset in bipolar disorder.	topic_bd
76859	1	355994	5	NULL	NULL	0	NULL	chemical fingerprint	Chemical		is present in					autistic children	GroupOfPeople				NULL	urine	0	NULL	NULL	NULL	NULL	NULL	Children with autism have a different chemical fingerprint in their urine than non-autistic children, according to new research published tomorrow in the print edition of the Journal of Proteome Research	topic_aut
76860	2	355994	5	NULL	NULL	0	NULL	chemical fingerprint	Chemical		is present in					non-autistic children	GroupOfPeople				NULL	urine	0	NULL	NULL	NULL	NULL	NULL	Children with autism have a different chemical fingerprint in their urine than non-autistic children, according to new research published tomorrow in the print edition of the Journal of Proteome Research	topic_aut
76861	3	355994	5	NULL	NULL	0	NULL	statement 1	Process		different from					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Children with autism have a different chemical fingerprint in their urine than non-autistic children, according to new research published tomorrow in the print edition of the Journal of Proteome Research	topic_aut
77438	1	355995	7	NULL	NULL	0	NULL	bipolar disorder	MedicalFinding	early onset of	increase		may			cannabis	Organism	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	This indicates that an early onset may increase the risk of cannabis use and that cannabis use may trigger bipolar disorder in vulnerable individuals.	topic_bd
77439	2	355995	7	NULL	NULL	0	NULL	cannabis	Organism		trigger		may			bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	This indicates that an early onset may increase the risk of cannabis use and that cannabis use may trigger bipolar disorder in vulnerable individuals.	topic_bd
76915	1	355996	5	NULL	NULL	NULL	NULL	diarrhea	MedicalFinding		is not associated with					ASDs	MedicalFinding				NULL	children	NULL	NULL	NULL	NULL	NULL	NULL	Parents of children and adolescents with autism spectrum disorders (ASDs) sometimes report that their children suffer from gastrointestinal (GI) symptoms, such as diarrhea and constipation. However, studies on how prevalent these symptoms are have had conflicting results.	topic_aut
76916	2	355996	5	NULL	NULL	NULL	NULL	diarrhea	MedicalFinding		is not associated with					ASDs	MedicalFinding				NULL	adolescents	NULL	NULL	NULL	NULL	NULL	NULL	Parents of children and adolescents with autism spectrum disorders (ASDs) sometimes report that their children suffer from gastrointestinal (GI) symptoms, such as diarrhea and constipation. However, studies on how prevalent these symptoms are have had conflicting results.	topic_aut
76917	3	355996	5	NULL	NULL	NULL	NULL	constipation	MedicalFinding		is not associated with					ASDs	MedicalFinding				NULL	children	NULL	NULL	NULL	NULL	NULL	NULL	Parents of children and adolescents with autism spectrum disorders (ASDs) sometimes report that their children suffer from gastrointestinal (GI) symptoms, such as diarrhea and constipation. However, studies on how prevalent these symptoms are have had conflicting results.	topic_aut
76918	4	355996	5	NULL	NULL	NULL	NULL	constipation	MedicalFinding		is not associated with					ASDs	MedicalFinding				NULL	adolescents	NULL	NULL	NULL	NULL	NULL	NULL	Parents of children and adolescents with autism spectrum disorders (ASDs) sometimes report that their children suffer from gastrointestinal (GI) symptoms, such as diarrhea and constipation. However, studies on how prevalent these symptoms are have had conflicting results.	topic_aut
76919	5	355996	5	NULL	NULL	0	NULL	ASDs	MedicalFinding		is					autism spectrum disorders	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Parents of children and adolescents with autism spectrum disorders (ASDs) sometimes report that their children suffer from gastrointestinal (GI) symptoms, such as diarrhea and constipation. However, studies on how prevalent these symptoms are have had conflicting results.	topic_aut
76920	6	355996	5	NULL	NULL	0	NULL	GI	OrganismPart		is					gastrointestinal	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Parents of children and adolescents with autism spectrum disorders (ASDs) sometimes report that their children suffer from gastrointestinal (GI) symptoms, such as diarrhea and constipation. However, studies on how prevalent these symptoms are have had conflicting results.	topic_aut
76921	7	355996	5	NULL	NULL	0	NULL	diarrhea	MedicalFinding		is a type of					GI symptom	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Parents of children and adolescents with autism spectrum disorders (ASDs) sometimes report that their children suffer from gastrointestinal (GI) symptoms, such as diarrhea and constipation. However, studies on how prevalent these symptoms are have had conflicting results.	topic_aut
76922	8	355996	5	NULL	NULL	0	NULL	constipation	MedicalFinding		is a type of					GI symptom	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Parents of children and adolescents with autism spectrum disorders (ASDs) sometimes report that their children suffer from gastrointestinal (GI) symptoms, such as diarrhea and constipation. However, studies on how prevalent these symptoms are have had conflicting results.	topic_aut
76923	1	355997	5	NULL	NULL	0	NULL	ASDs	MedicalFinding		is					autism spectrum disorders	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Reports have suggested that sleep problems in children and adolescents with autism spectrum disorders (ASDs) are associated with challenging daytime behaviors.	topic_aut
76924	2	355997	5	NULL	NULL	0	NULL	ASDs children	GroupOfPeople		suffer from					sleep problems	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Reports have suggested that sleep problems in children and adolescents with autism spectrum disorders (ASDs) are associated with challenging daytime behaviors.	topic_aut
76925	3	355997	5	NULL	NULL	0	NULL	statement 2	Process		is associated with					daytime behaviors	MentalProcess	challenging			NULL		0	NULL	NULL	NULL	NULL	NULL	Reports have suggested that sleep problems in children and adolescents with autism spectrum disorders (ASDs) are associated with challenging daytime behaviors.	topic_aut
76926	4	355997	5	NULL	NULL	0	NULL	ASDs adolescents	GroupOfPeople		suffer from					sleep problems	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Reports have suggested that sleep problems in children and adolescents with autism spectrum disorders (ASDs) are associated with challenging daytime behaviors.	topic_aut
76927	5	355997	5	NULL	NULL	0	NULL	statement 4	Process		is associated with					daytime behaviors	MentalProcess	challenging			NULL		0	NULL	NULL	NULL	NULL	NULL	Reports have suggested that sleep problems in children and adolescents with autism spectrum disorders (ASDs) are associated with challenging daytime behaviors.	topic_aut
77440	1	355998	7	NULL	NULL	0	NULL	neuroplasticity	MedicalFinding	changes in	neuropathological findings in					BD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Recent data suggest that changes in neuroplasticity, cell resilience and connectivity are the main neuropathological findings in BD.	topic_bd
77441	2	355998	7	NULL	NULL	0	NULL	cell resilience	Process	changes in	neuropathological findings in					BD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Recent data suggest that changes in neuroplasticity, cell resilience and connectivity are the main neuropathological findings in BD.	topic_bd
77442	3	355998	7	NULL	NULL	NULL	NULL	cell connectivity 	Process	changes in	neuropathological findings in					BD	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Recent data suggest that changes in neuroplasticity, cell resilience and connectivity are the main neuropathological findings in BD.	topic_bd
77443	1	355999	7	NULL	NULL	0	NULL	nephrotic syndrome	MedicalFinding		occur during					 induction chemotherapy	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	This report is the first to document minimal change nephrotic syndrome occurring during induction chemotherapy for childhood acute lymphoblastic leukemia (ALL). 	topic_ll
77444	2	355999	7	NULL	NULL	0	NULL	statement 1	Process		occur upon					ALL	MedicalFinding	childhood			NULL		0	NULL	NULL	NULL	NULL	NULL	This report is the first to document minimal change nephrotic syndrome occurring during induction chemotherapy for childhood acute lymphoblastic leukemia (ALL). 	topic_ll
77445	3	355999	7	NULL	NULL	0	NULL	ALL	MedicalFinding		is					acute lymphoblastic leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	This report is the first to document minimal change nephrotic syndrome occurring during induction chemotherapy for childhood acute lymphoblastic leukemia (ALL). 	topic_ll
77446	1	356001	7	NULL	NULL	0	NULL	immune cell dysregulation	Process		central to					nephrotic syndrome	MedicalFinding	pathogenesis of			NULL		0	NULL	NULL	NULL	NULL	NULL	This occurrence lends further support to the theory of immune cell dysregulation being central to the pathogenesis of nephrotic syndrome in ALL	topic_ll
77447	2	356001	7	NULL	NULL	0	NULL	statement 1	Process		occur in					ALL	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	This occurrence lends further support to the theory of immune cell dysregulation being central to the pathogenesis of nephrotic syndrome in ALL	topic_ll
77448	1	356002	7	NULL	NULL	0	NULL	GSK-3	GP		helps in					apoptosis	Process	regulating			NULL		0	NULL	NULL	NULL	NULL	NULL	Among many other things, GSK-3 helps regulate programmed cell death (apoptosis).	topic_bd
77449	2	356002	7	NULL	NULL	0	NULL	apoptosis	Process		is					programmed cell death	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Among many other things, GSK-3 helps regulate programmed cell death (apoptosis).	topic_bd
76928	1	356003	5	NULL	NULL	0	NULL	healthy children	GroupOfPeople		deficient in					tryptophan	AminoAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	This method is precise and sensitive for the detection of low concentrations of tryptophan and can be applicable to monitoring its level in human urine. Children with autism have a higher deficiency of tryptophan than the control group of healthy children	topic_aut
76929	2	356003	5	NULL	NULL	0	NULL	autistic children	GroupOfPeople		deficient in					tryptophan	AminoAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	This method is precise and sensitive for the detection of low concentrations of tryptophan and can be applicable to monitoring its level in human urine. Children with autism have a higher deficiency of tryptophan than the control group of healthy children	topic_aut
76930	3	356003	5	NULL	NULL	0	NULL	statement 2	Process		is higher than					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	This method is precise and sensitive for the detection of low concentrations of tryptophan and can be applicable to monitoring its level in human urine. Children with autism have a higher deficiency of tryptophan than the control group of healthy children	topic_aut
76931	1	356004	5	NULL	NULL	0	NULL	depression	MedicalFinding	mild	is a symptom of					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Lower levels of tryptophan may lead to the worsening of autistic symptoms such as mild depression and increased irritability.	topic_aut
76932	2	356004	5	NULL	NULL	0	NULL	irritability	MedicalFinding	increased	is a symptom of					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Lower levels of tryptophan may lead to the worsening of autistic symptoms such as mild depression and increased irritability.	topic_aut
76933	3	356004	5	NULL	NULL	0	NULL	tryptophan	AminoAcid	lower levels of	worsens					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Lower levels of tryptophan may lead to the worsening of autistic symptoms such as mild depression and increased irritability.	topic_aut
76934	4	356004	5	NULL	NULL	0	NULL	tryptophan	AminoAcid	lower levels of	worsens					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Lower levels of tryptophan may lead to the worsening of autistic symptoms such as mild depression and increased irritability.	topic_aut
76959	1	356005	5	NULL	NULL	0	NULL	HVA	Chemical		is present in					autistic children	GroupOfPeople	urine of			NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of HVA and VMA were higher in the urine of autistic children (28.8+/-15.5 micromol/mmol creatinine and 22.2+/-13.0 micromol/mmol creatinine, respectively) compared with those of the generally healthy children (4.6+/-0.7 micromol/mmol creatinine for HVA and 3.8+/-0.6 micromol/mmol creatinine for VMA).	topic_aut
76960	2	356005	5	NULL	NULL	0	NULL	HVA	Chemical		is present in					healthy children	GroupOfPeople	urine of			NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of HVA and VMA were higher in the urine of autistic children (28.8+/-15.5 micromol/mmol creatinine and 22.2+/-13.0 micromol/mmol creatinine, respectively) compared with those of the generally healthy children (4.6+/-0.7 micromol/mmol creatinine for HVA and 3.8+/-0.6 micromol/mmol creatinine for VMA).	topic_aut
76961	3	356005	5	NULL	NULL	0	NULL	statement 1	Process	level of	is higher than					statement 2	Process	levels of			NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of HVA and VMA were higher in the urine of autistic children (28.8+/-15.5 micromol/mmol creatinine and 22.2+/-13.0 micromol/mmol creatinine, respectively) compared with those of the generally healthy children (4.6+/-0.7 micromol/mmol creatinine for HVA and 3.8+/-0.6 micromol/mmol creatinine for VMA).	topic_aut
76962	4	356005	5	NULL	NULL	0	NULL	VMA	Chemical		is present in					autistic children	GroupOfPeople	urine of			NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of HVA and VMA were higher in the urine of autistic children (28.8+/-15.5 micromol/mmol creatinine and 22.2+/-13.0 micromol/mmol creatinine, respectively) compared with those of the generally healthy children (4.6+/-0.7 micromol/mmol creatinine for HVA and 3.8+/-0.6 micromol/mmol creatinine for VMA).	topic_aut
76963	5	356005	5	NULL	NULL	0	NULL	VMA	Chemical		is present in					healthy children	GroupOfPeople	urine of			NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of HVA and VMA were higher in the urine of autistic children (28.8+/-15.5 micromol/mmol creatinine and 22.2+/-13.0 micromol/mmol creatinine, respectively) compared with those of the generally healthy children (4.6+/-0.7 micromol/mmol creatinine for HVA and 3.8+/-0.6 micromol/mmol creatinine for VMA).	topic_aut
76964	6	356005	5	NULL	NULL	0	NULL	statement 4	Process	level of	is higher than					statement 5	Process	level of			NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of HVA and VMA were higher in the urine of autistic children (28.8+/-15.5 micromol/mmol creatinine and 22.2+/-13.0 micromol/mmol creatinine, respectively) compared with those of the generally healthy children (4.6+/-0.7 micromol/mmol creatinine for HVA and 3.8+/-0.6 micromol/mmol creatinine for VMA).	topic_aut
76965	1	356006	5	NULL	NULL	0	NULL	dopamine metabolism disorder	MedicalFinding		is present in					autistic children	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of urinary homovanillic acid (HVA) and vanillylmandelic acid (VMA) can be a very important tool in the study of disorders of dopamine metabolism in autistic children	topic_aut
76966	2	356006	5	NULL	NULL	NULL	NULL	HVA	Chemical	quantification of;;urinary	plays a role in		may			statement 1	Process	study of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Quantification of urinary homovanillic acid (HVA) and vanillylmandelic acid (VMA) can be a very important tool in the study of disorders of dopamine metabolism in autistic children	topic_aut
76967	3	356006	5	NULL	NULL	NULL	NULL	VMA	Chemical	quantification of;;urinary	plays a role in		may			statement 1	Process	study of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Quantification of urinary homovanillic acid (HVA) and vanillylmandelic acid (VMA) can be a very important tool in the study of disorders of dopamine metabolism in autistic children	topic_aut
76968	4	356006	5	NULL	NULL	0	NULL	VMA	Chemical		is					vanillylmandelic acid	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of urinary homovanillic acid (HVA) and vanillylmandelic acid (VMA) can be a very important tool in the study of disorders of dopamine metabolism in autistic children	topic_aut
76969	5	356006	5	NULL	NULL	0	NULL	HVA	Chemical		is					homovanillic acid	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of urinary homovanillic acid (HVA) and vanillylmandelic acid (VMA) can be a very important tool in the study of disorders of dopamine metabolism in autistic children	topic_aut
76970	1	356007	5	NULL	NULL	0	NULL	VMA	Chemical		is					Vanillyl mandelic acid	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Vanillyl mandelic acid (VMA) is an end-stage metabolite of the catecholamines epinephrine and norepinephrine. It is produced via intermediary metabolites	topic_aut
76971	2	356007	5	NULL	NULL	0	NULL	epinephrine	Chemical		is a type of					catecholamines	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Vanillyl mandelic acid (VMA) is an end-stage metabolite of the catecholamines epinephrine and norepinephrine. It is produced via intermediary metabolites	topic_aut
76972	3	356007	5	NULL	NULL	0	NULL	norepinephrine	Chemical		is a type of					catecholamines	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Vanillyl mandelic acid (VMA) is an end-stage metabolite of the catecholamines epinephrine and norepinephrine. It is produced via intermediary metabolites	topic_aut
76973	4	356007	5	NULL	NULL	0	NULL	VMA	Chemical		is an end-stage metabolite of					epinephrine	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Vanillyl mandelic acid (VMA) is an end-stage metabolite of the catecholamines epinephrine and norepinephrine. It is produced via intermediary metabolites	topic_aut
76974	5	356007	5	NULL	NULL	0	NULL	VMA	Chemical		is an end-stage metabolite of					norepinephrine	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Vanillyl mandelic acid (VMA) is an end-stage metabolite of the catecholamines epinephrine and norepinephrine. It is produced via intermediary metabolites	topic_aut
76975	1	356008	5	NULL	NULL	0	NULL	(HOC6H3(OCH3)CH2COOH	Chemical		is					Homovanillic acid	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Homovanillic acid (HOC6H3(OCH3)CH2COOH;  is a major catecholamine metabolite.	topic_aut
76976	2	356008	5	NULL	NULL	0	NULL	Homovanillic acid	Chemical		is a metabolite of					catecholamine	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Homovanillic acid (HOC6H3(OCH3)CH2COOH;  is a major catecholamine metabolite.	topic_aut
76977	1	356009	5	NULL	NULL	0	NULL	ASD	MedicalFinding		is					autistic spectrum disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Insomnia is the predominant sleep concern in children with autistic spectrum disorder (ASD)	topic_aut
76978	2	356009	5	NULL	NULL	0	NULL	Insomnia	MedicalFinding		is a symptom of					ASD children	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Insomnia is the predominant sleep concern in children with autistic spectrum disorder (ASD)	topic_aut
76984	1	356010	5	NULL	NULL	NULL	NULL	melatonin	GP	low concentration of	is caused by					acetylserotonin methyltransferase activity	Process	primary deficit in			NULL		NULL	NULL	NULL	NULL	NULL	NULL	A recent study using a combination of genetic and functional experimental techniques reported evidence that low melatonin concentration caused by a primary deficit in acetylserotonin methyltransferase activity is a risk factor for ASD	topic_aut
76998	2	356010	5	NULL	NULL	0	NULL	statement 1	Process		is a risk factor for					ASD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	A recent study using a combination of genetic and functional experimental techniques reported evidence that low melatonin concentration caused by a primary deficit in acetylserotonin methyltransferase activity is a risk factor for ASD	topic_aut
76999	1	356011	5	NULL	NULL	NULL	NULL	repetitive behavior	MedicalFinding		is a symptom of					autism spectrum disorders	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Results of this trial do not support the use of citalopram for the treatment of repetitive behavior in children and adolescents with autism spectrum disorders	topic_aut
77000	2	356011	5	NULL	NULL	NULL	NULL	citalopram	Chemical		does not treat					statement 1	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Results of this trial do not support the use of citalopram for the treatment of repetitive behavior in children and adolescents with autism spectrum disorders	topic_aut
77001	3	356011	5	NULL	NULL	0	NULL	statement 1	MedicalFinding		occurs in					children	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Results of this trial do not support the use of citalopram for the treatment of repetitive behavior in children and adolescents with autism spectrum disorders	topic_aut
77002	4	356011	5	NULL	NULL	0	NULL	statement 2	MedicalFinding		occurs in					adolescents	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Results of this trial do not support the use of citalopram for the treatment of repetitive behavior in children and adolescents with autism spectrum disorders	topic_aut
77451	1	356012	7	NULL	NULL	0	NULL	memantine	Chemical		have		may			antimanic properties	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Memantine may have antimanic properties.	topic_bd
78059	1	356015	6	NULL	NULL	NULL	NULL	 zoledronic acid	Chemical		improves					premenopausal patients	Person	survival of 			NULL		NULL	NULL	NULL	NULL	NULL	NULL	The addition of zoledronic acid to adjuvant endocrine therapy improves disease-free survival in premenopausal patients with estrogen-responsive early breast cancer.	topic_bc
78181	1	356016	6	NULL	NULL	0	NULL	tamoxifen	Chemical		decrease					Breast cancer	MedicalFinding	mortality from			NULL		0	NULL	NULL	NULL	NULL	NULL	Endocrine therapies targeting oestrogen action (anti-oestrogens, such as tamoxifen, and aromatase inhibitors) decrease mortality from breast cancer, but their efficacy is limited by intrinsic and acquired therapeutic resistance.	topic_bc
78182	2	356016	6	NULL	NULL	0	NULL	aromatase inhibitor	Chemical		decrease					Breast cancer	MedicalFinding	mortality from			NULL		0	NULL	NULL	NULL	NULL	NULL	Endocrine therapies targeting oestrogen action (anti-oestrogens, such as tamoxifen, and aromatase inhibitors) decrease mortality from breast cancer, but their efficacy is limited by intrinsic and acquired therapeutic resistance.	topic_bc
78183	3	356016	6	NULL	NULL	0	NULL	tamoxifen	Chemical		is a type of					anti-estrogen	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Endocrine therapies targeting oestrogen action (anti-oestrogens, such as tamoxifen, and aromatase inhibitors) decrease mortality from breast cancer, but their efficacy is limited by intrinsic and acquired therapeutic resistance.	topic_bc
78184	4	356016	6	NULL	NULL	0	NULL	aromatase inhibitor	Chemical		is a type of					anti-oestrogen	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Endocrine therapies targeting oestrogen action (anti-oestrogens, such as tamoxifen, and aromatase inhibitors) decrease mortality from breast cancer, but their efficacy is limited by intrinsic and acquired therapeutic resistance.	topic_bc
78060	1	356017	6	NULL	NULL	0	NULL	Oestrogen	Chemical		causes					epithelium	OrganismPart	hyperproliferation of			NULL		0	NULL	NULL	NULL	NULL	NULL	Oestrogen predominance over progesterone may cause hyperproliferation of mammary epithelium and thus promote breast carcinogenesis.	topic_bc
78061	2	356017	6	NULL	NULL	0	NULL	statement 1	process		promotes					breast carcinoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Oestrogen predominance over progesterone may cause hyperproliferation of mammary epithelium and thus promote breast carcinogenesis.	topic_bc
77452	1	356019	7	NULL	NULL	0	NULL	RUNX1	GP		known as					CBFA2 	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	RUNX1, also known as CBFA2 (core binding factor A2)	topic_ll
77453	2	356019	7	NULL	NULL	0	NULL	CBFA2	GP		is					core binding factor A2	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	RUNX1, also known as CBFA2 (core binding factor A2)	topic_ll
77003	1	356020	5	NULL	NULL	0	NULL	gene loci	Chromosome	different	is located on					6p22.1	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	Recently, genetic data from multiple large cohorts of patients were published in ‘Nature’ showing that different gene loci located on chromosome 6p22.1 are the most probable susceptibility genes for schizophrenia (Shi et al., 2009; Stefansson et al., 2009; Purcell et al., 2009). NULL	topic_sch
77004	2	356020	5	NULL	NULL	NULL	NULL	statement 1	Chromosome		susceptibile to		most probable			schizophrenia	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Recently, genetic data from multiple large cohorts of patients were published in ‘Nature’ showing that different gene loci located on chromosome 6p22.1 are the most probable susceptibility genes for schizophrenia (Shi et al., 2009; Stefansson et al., 2009; Purcell et al., 2009). NULL	topic_sch
77005	1	356022	5	NULL	NULL	0	NULL	genes	GP		is present in					HLA complex	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, several genes of the HLA complex, which regulate the immune function and already earlier have been discussed to be involved in schizophrenia, are located in these regions (Fellerhoff et al., 2007). 	topic_sch
77006	2	356022	5	NULL	NULL	0	NULL	statement 1	GP		regulates					immune function	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, several genes of the HLA complex, which regulate the immune function and already earlier have been discussed to be involved in schizophrenia, are located in these regions (Fellerhoff et al., 2007). 	topic_sch
77007	3	356022	5	NULL	NULL	0	NULL	statement 1	GP		is involved in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, several genes of the HLA complex, which regulate the immune function and already earlier have been discussed to be involved in schizophrenia, are located in these regions (Fellerhoff et al., 2007). 	topic_sch
77008	1	356024	5	NULL	NULL	0	NULL	IL-8	GP		is					Interleukin-8	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	In humans it could be shown that increased maternal levels of the pro-inflammatory cytokine Interleukin-8 (IL-8) during pregnancy are associated with an increased risk for schizophrenia in the offspring – whatever the reason for increased IL-8 was (Brown, 2006).	topic_sch
77009	2	356024	5	NULL	NULL	0	NULL	IL-8	GP		is a type of					pro-inflammatory cytokine	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	In humans it could be shown that increased maternal levels of the pro-inflammatory cytokine Interleukin-8 (IL-8) during pregnancy are associated with an increased risk for schizophrenia in the offspring – whatever the reason for increased IL-8 was (Brown, 2006).	topic_sch
77010	3	356024	5	NULL	NULL	0	NULL	IL-8	GP	increase in;;levels of;;maternal	occurs during					pregnancy	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	In humans it could be shown that increased maternal levels of the pro-inflammatory cytokine Interleukin-8 (IL-8) during pregnancy are associated with an increased risk for schizophrenia in the offspring – whatever the reason for increased IL-8 was (Brown, 2006).	topic_sch
77011	4	356024	5	NULL	NULL	0	NULL	statement 3	Process		is associated with					schizophrenia	MedicalFinding	increased risk for			NULL		0	NULL	NULL	NULL	NULL	NULL	In humans it could be shown that increased maternal levels of the pro-inflammatory cytokine Interleukin-8 (IL-8) during pregnancy are associated with an increased risk for schizophrenia in the offspring – whatever the reason for increased IL-8 was (Brown, 2006).	topic_sch
77012	5	356024	5	NULL	NULL	0	NULL	statement 4	Process		occurs in					offspring	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	In humans it could be shown that increased maternal levels of the pro-inflammatory cytokine Interleukin-8 (IL-8) during pregnancy are associated with an increased risk for schizophrenia in the offspring – whatever the reason for increased IL-8 was (Brown, 2006).	topic_sch
77013	1	356025	5	NULL	NULL	0	NULL	mother	GroupOfPeople	immune response of	is related to		may be			schizophrenia	MedicalFinding	increased risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	As opposed to any single pathogen, the immune response, itself, of the mother may be related to the increased risk for schizophrenia in the offspring (Zuckerman and Weiner, 2005).	topic_sch
77014	2	356025	5	NULL	NULL	0	NULL	statement 1	Process		occurs in					offspring	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	As opposed to any single pathogen, the immune response, itself, of the mother may be related to the increased risk for schizophrenia in the offspring (Zuckerman and Weiner, 2005).	topic_sch
77015	1	356026	5	NULL	NULL	NULL	NULL	CNS	OrganismPart		infected during					childhood	Time	early			NULL		NULL	NULL	NULL	NULL	NULL	NULL	A five-fold increased risk for developing psychoses later on, however, was detected after infection of the CNS in early childhood (Brown et al., 2004; Gattaz et al., 2004).	topic_sch
77016	2	356026	5	NULL	NULL	0	NULL	statement 1	Process		increases					psychoses	MedicalFinding	risk of;;development of			NULL		0	NULL	NULL	NULL	NULL	NULL	A five-fold increased risk for developing psychoses later on, however, was detected after infection of the CNS in early childhood (Brown et al., 2004; Gattaz et al., 2004).	topic_sch
77017	1	356027	5	NULL	NULL	0	NULL	inflammation	MedicalFinding	signs of	is present in					brain	OrganismPart	schizophrenic			NULL		0	NULL	NULL	NULL	NULL	NULL	Signs of inflammation were found in schizophrenic brains (Körschenhausen et al., 1996), and the term ‘mild localized chronic encephalitis’ to describe a slight but chronic inflammatory process in schizophrenia was proposed (Bechter, 2001). 	topic_sch
77018	2	356027	5	NULL	NULL	0	NULL	inflammatory process	MedicalFinding	slight;;chronic	is observed in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Signs of inflammation were found in schizophrenic brains (Körschenhausen et al., 1996), and the term ‘mild localized chronic encephalitis’ to describe a slight but chronic inflammatory process in schizophrenia was proposed (Bechter, 2001). 	topic_sch
77019	3	356027	5	NULL	NULL	0	NULL	statement 2	Process		is termed as					mild localized chronic encephalitis	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Signs of inflammation were found in schizophrenic brains (Körschenhausen et al., 1996), and the term ‘mild localized chronic encephalitis’ to describe a slight but chronic inflammatory process in schizophrenia was proposed (Bechter, 2001). 	topic_sch
77020	1	356028	5	NULL	NULL	NULL	NULL	IL-2	GP	decreased;;production of	reflects					type-1 cytokines	GP	blunted production of			NULL	in vitro	NULL	NULL	NULL	NULL	NULL	NULL	A well established finding in schizophrenia is the decreased in vitro production of IL-2 and IFN-! (Wilke et al., 1996; Müller et al., 2000), reflecting a blunted production of type-1 cytokines	topic_sch
77021	2	356028	5	NULL	NULL	NULL	NULL	IFN-gamma	GP	decreased;;production of	reflects					type-1 cytokines	GP	blunted production of			NULL	in vitro	NULL	NULL	NULL	NULL	NULL	NULL	A well established finding in schizophrenia is the decreased in vitro production of IL-2 and IFN-! (Wilke et al., 1996; Müller et al., 2000), reflecting a blunted production of type-1 cytokines	topic_sch
77022	3	356028	5	NULL	NULL	0	NULL	statement 1	Process		occurs in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	A well established finding in schizophrenia is the decreased in vitro production of IL-2 and IFN-! (Wilke et al., 1996; Müller et al., 2000), reflecting a blunted production of type-1 cytokines	topic_sch
77023	4	356028	5	NULL	NULL	0	NULL	statement 2	Process		occurs in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	A well established finding in schizophrenia is the decreased in vitro production of IL-2 and IFN-! (Wilke et al., 1996; Müller et al., 2000), reflecting a blunted production of type-1 cytokines	topic_sch
77454	1	356029	7	NULL	NULL	0	NULL	p-STAT3	GP	overexpression of	associated with		significantly			colorectal cancer-specific mortality	Process	higher			NULL		0	NULL	NULL	NULL	NULL	NULL	 p-STAT3 overexpression was associated with significantly higher colorectal cancer-specific mortality	topic_ccc
77455	1	356030	7	NULL	NULL	0	NULL	Preoperative serum p53 Abs 	GP		not marker for					tumor 	MedicalFinding	progression of			NULL		0	NULL	NULL	NULL	NULL	NULL	Preoperative serum p53 Abs do not seem to be a marker of tumor progression but may be a useful marker for detecting high risk of lymph node metastasis in T1 colorectal cancer.	topic_ccc
77456	2	356030	7	NULL	NULL	0	NULL	Preoperative serum p53 Abs 	GP		marker for		useful			lymph node metastasis	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Preoperative serum p53 Abs do not seem to be a marker of tumor progression but may be a useful marker for detecting high risk of lymph node metastasis in T1 colorectal cancer.	topic_ccc
77457	3	356030	7	NULL	NULL	0	NULL	statement 2	Process		occur in					T1 colorectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Preoperative serum p53 Abs do not seem to be a marker of tumor progression but may be a useful marker for detecting high risk of lymph node metastasis in T1 colorectal cancer.	topic_ccc
77458	1	356031	7	NULL	NULL	0	NULL	MSH2 	GP	mutations of	underlie					hereditary non-polyposis colorectal cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the mismatch repair gene MSH2 underlie hereditary non-polyposis colorectal cancer (Lynch syndrome)	topic_ccc
77459	2	356031	7	NULL	NULL	0	NULL	MSH2	GP		is a type of					mismatch repair gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the mismatch repair gene MSH2 underlie hereditary non-polyposis colorectal cancer (Lynch syndrome)	topic_ccc
77460	3	356031	7	NULL	NULL	0	NULL	hereditary non-polyposis colorectal cancer	MedicalFinding		is					Lynch syndrome	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the mismatch repair gene MSH2 underlie hereditary non-polyposis colorectal cancer (Lynch syndrome)	topic_ccc
77461	1	356032	7	NULL	NULL	0	NULL	MSH2	GP	mutations of	underlie					hereditary non-polyposis colorectal cancer 	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the mismatch repair gene MSH2 underlie hereditary non-polyposis colorectal cancer (Lynch syndrome). While disruptive mutations are overtly pathogenic, the implications of missense mutations found in sporadic colorectal cancer patients or in suspected Lynch syndrome families are often unknown.	topic_ccc
77462	2	356032	7	NULL	NULL	0	NULL	hereditary non-polyposis colorectal cancer 	MedicalFinding		is					Lynch syndrome	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the mismatch repair gene MSH2 underlie hereditary non-polyposis colorectal cancer (Lynch syndrome). While disruptive mutations are overtly pathogenic, the implications of missense mutations found in sporadic colorectal cancer patients or in suspected Lynch syndrome families are often unknown.	topic_ccc
77463	3	356032	7	NULL	NULL	0	NULL	MSH2	GP	disruptive mutations of	are					pathogenic	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the mismatch repair gene MSH2 underlie hereditary non-polyposis colorectal cancer (Lynch syndrome). While disruptive mutations are overtly pathogenic, the implications of missense mutations found in sporadic colorectal cancer patients or in suspected Lynch syndrome families are often unknown.	topic_ccc
77464	4	356032	7	NULL	NULL	0	NULL	missense mutations 	Process		found in					sporadic colorectal cancer 	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the mismatch repair gene MSH2 underlie hereditary non-polyposis colorectal cancer (Lynch syndrome). While disruptive mutations are overtly pathogenic, the implications of missense mutations found in sporadic colorectal cancer patients or in suspected Lynch syndrome families are often unknown.	topic_ccc
77465	5	356032	7	NULL	NULL	0	NULL	missense mutations	Process		found in					suspected Lynch syndrome families	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the mismatch repair gene MSH2 underlie hereditary non-polyposis colorectal cancer (Lynch syndrome). While disruptive mutations are overtly pathogenic, the implications of missense mutations found in sporadic colorectal cancer patients or in suspected Lynch syndrome families are often unknown.	topic_ccc
77484	6	356032	7	NULL	NULL	0	NULL	MSH2	GP		is a type of					mismatch repair gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the mismatch repair gene MSH2 underlie hereditary non-polyposis colorectal cancer (Lynch syndrome). While disruptive mutations are overtly pathogenic, the implications of missense mutations found in sporadic colorectal cancer patients or in suspected Lynch syndrome families are often unknown.	topic_ccc
77024	1	356033	5	NULL	NULL	0	NULL	autism	MedicalFinding		is characterized by					social relatedness	MentalProcess	core impairments of			NULL		0	NULL	NULL	NULL	NULL	NULL	Autism is characterized by core impairments in social relatedness and communication and interfering repetitive behaviors	topic_aut
77025	2	356033	5	NULL	NULL	0	NULL	autism	MedicalFinding		is characterized by					communication	MentalProcess	core impairments of			NULL		0	NULL	NULL	NULL	NULL	NULL	Autism is characterized by core impairments in social relatedness and communication and interfering repetitive behaviors	topic_aut
77026	3	356033	5	NULL	NULL	0	NULL	autism	MedicalFinding		is characterized by					interfering repetitive behaviors	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Autism is characterized by core impairments in social relatedness and communication and interfering repetitive behaviors	topic_aut
77027	1	356035	5	NULL	NULL	0	NULL	5-hydroxytryptophan	Chemical	daily treatment with	clinically improves					5HIAA	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	Daily treatment with 5-hydroxytryptophan (and carbidopa) led to clinical improvement and normalization of 5HIAA, implying that brain serotonin turnover normalized	topic_aut
77028	2	356035	5	NULL	NULL	0	NULL	5-hydroxytryptophan	Chemical	daily treatment with	normalize					5HIAA	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Daily treatment with 5-hydroxytryptophan (and carbidopa) led to clinical improvement and normalization of 5HIAA, implying that brain serotonin turnover normalized	topic_aut
77029	3	356035	5	NULL	NULL	NULL	NULL	carbidopa	Chemical	daily treatment with	clinically improves					5HIAA	Chemical				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Daily treatment with 5-hydroxytryptophan (and carbidopa) led to clinical improvement and normalization of 5HIAA, implying that brain serotonin turnover normalized	topic_aut
77030	4	356035	5	NULL	NULL	0	NULL	carbidopa	Chemical	daily treatment with	normalize					5HIAA	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Daily treatment with 5-hydroxytryptophan (and carbidopa) led to clinical improvement and normalization of 5HIAA, implying that brain serotonin turnover normalized	topic_aut
77031	5	356035	5	NULL	NULL	0	NULL	statement 1	Process		imply					serotonin	GP	normalized turnover of;;brain			NULL		0	NULL	NULL	NULL	NULL	NULL	Daily treatment with 5-hydroxytryptophan (and carbidopa) led to clinical improvement and normalization of 5HIAA, implying that brain serotonin turnover normalized	topic_aut
77032	6	356035	5	NULL	NULL	0	NULL	statement 2	Process		imply					serotonin	GP	normalized turnover of;;brain			NULL		0	NULL	NULL	NULL	NULL	NULL	Daily treatment with 5-hydroxytryptophan (and carbidopa) led to clinical improvement and normalization of 5HIAA, implying that brain serotonin turnover normalized	topic_aut
77033	7	356035	5	NULL	NULL	0	NULL	statement 3	Process		imply					serotonin	GP	normalized turnover of;;brain			NULL		0	NULL	NULL	NULL	NULL	NULL	Daily treatment with 5-hydroxytryptophan (and carbidopa) led to clinical improvement and normalization of 5HIAA, implying that brain serotonin turnover normalized	topic_aut
77034	8	356035	5	NULL	NULL	0	NULL	statement 4	Process		imply					serotonin	GP	normalized turnover of;;brain			NULL		0	NULL	NULL	NULL	NULL	NULL	Daily treatment with 5-hydroxytryptophan (and carbidopa) led to clinical improvement and normalization of 5HIAA, implying that brain serotonin turnover normalized	topic_aut
77466	1	356036	7	NULL	NULL	0	NULL	IDH2	GP	overexpression of;;wild-type	increase		significantly			 5-methylcytosine 	Chemical	levels of			NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of wild-type IDH2 also led to a small but significant increase in 5-methylcytosine levels compared to vector control, consistent with the small 2HG elevation observed in these cells.	topic_ll
77467	2	356036	7	NULL	NULL	0	NULL	IDH2	GP	overexpression of;;wild-type	elevates					2HG	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of wild-type IDH2 also led to a small but significant increase in 5-methylcytosine levels compared to vector control, consistent with the small 2HG elevation observed in these cells.	topic_ll
77468	1	356037	7	NULL	NULL	NULL	NULL	GATA1 	GP		hypermethylated in		aberrantly			IDH1-mutant AMLs	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	GATA1 was aberrantly hypermethylated and silenced specifically in IDH1-mutant AMLs 	topic_ll
77469	2	356037	7	NULL	NULL	0	NULL	GATA1	GP		silenced in		specifically			IDH1-mutant AMLs	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	GATA1 was aberrantly hypermethylated and silenced specifically in IDH1-mutant AMLs 	topic_ll
77470	1	356038	7	NULL	NULL	0	NULL	TET2	GP	mutations in	constitute					AML	MedicalFinding	distinct mutational class in			NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that TET2 and IDH1/2 mutations constitute a distinct mutational class in AML which affects the epigenetic state	topic_ll
77471	2	356038	7	NULL	NULL	0	NULL	statement 1	Process		affects					epigenetic state	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that TET2 and IDH1/2 mutations constitute a distinct mutational class in AML which affects the epigenetic state	topic_ll
77472	3	356038	7	NULL	NULL	0	NULL	IDH1/2 	GP	mutations in	constitute					AML	MedicalFinding	distinct mutational class in			NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that TET2 and IDH1/2 mutations constitute a distinct mutational class in AML which affects the epigenetic state	topic_ll
77473	4	356038	7	NULL	NULL	0	NULL	statement 3			affects					epigenetic state	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that TET2 and IDH1/2 mutations constitute a distinct mutational class in AML which affects the epigenetic state	topic_ll
77474	1	356039	7	NULL	NULL	NULL	NULL	IDH1/ 2 	GP	expression of;;mutant	induce					DNA hypermethylation	Process	increase in;;global			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Most importantly, expression of IDH1/ 2 mutants induced an increase in global DNA hypermethylation, and inhibited TET2-induced cytosine 5-hydroxymethylation.	topic_ll
77475	2	356039	7	NULL	NULL	0	NULL	TET2	GP		induce					cytosine 5-hydroxymethylation	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Most importantly, expression of IDH1/ 2 mutants induced an increase in global DNA hypermethylation, and inhibited TET2-induced cytosine 5-hydroxymethylation.	topic_ll
77476	3	356039	7	NULL	NULL	0	NULL	IDH1/ 2	GP	expression of;;mutant	inhibit					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Most importantly, expression of IDH1/ 2 mutants induced an increase in global DNA hypermethylation, and inhibited TET2-induced cytosine 5-hydroxymethylation.	topic_ll
77477	1	356040	7	NULL	NULL	0	NULL	TET2	GP		hydroxylates					5-methylcytosine 	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	expression of mutant IDH is able to inhibit the hydroxylation of 5-methylcytosine by TET2 and subsequent DNA demethylation.	topic_ll
77478	2	356040	7	NULL	NULL	0	NULL	IDH	GP	expression of;;mutant	inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	expression of mutant IDH is able to inhibit the hydroxylation of 5-methylcytosine by TET2 and subsequent DNA demethylation.	topic_ll
77479	3	356040	7	NULL	NULL	0	NULL	statement 2	Process		demethylates		subsequently			DNA	NucleicAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	expression of mutant IDH is able to inhibit the hydroxylation of 5-methylcytosine by TET2 and subsequent DNA demethylation.	topic_ll
77480	1	356042	7	NULL	NULL	NULL	NULL	Down syndrome	MedicalFinding	children with	risk of		increased			AMKL	MedicalFinding	developing			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Children with constitutional trisomy 21 (Down syndrome) have an approximately 500-fold increased risk of developing acute megakaryoblastic leukemia (AMKL), a form of acute myeloid leukemia.	topic_ll
77481	2	356042	7	NULL	NULL	0	NULL	AMKL	MedicalFinding		is					acute megakaryoblastic leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Children with constitutional trisomy 21 (Down syndrome) have an approximately 500-fold increased risk of developing acute megakaryoblastic leukemia (AMKL), a form of acute myeloid leukemia.	topic_ll
77482	3	356042	7	NULL	NULL	0	NULL	AMKL	MedicalFinding		is a type of					acute myeloid leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Children with constitutional trisomy 21 (Down syndrome) have an approximately 500-fold increased risk of developing acute megakaryoblastic leukemia (AMKL), a form of acute myeloid leukemia.	topic_ll
77483	4	356042	7	NULL	NULL	0	NULL	Down syndrome	MedicalFinding		is					constitutional trisomy 21	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Children with constitutional trisomy 21 (Down syndrome) have an approximately 500-fold increased risk of developing acute megakaryoblastic leukemia (AMKL), a form of acute myeloid leukemia.	topic_ll
77485	1	356043	7	NULL	NULL	0	NULL	Down syndrome	MedicalFinding	newborn infants with	have					TL	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Unique to newborn infants with Down syndrome is a transient leukemia (TL), also referred to as transient myeloproliferative syn- drome, that undergoes spontaneous re-mission in the majority of cases but in approximately 20% is followed by AMKL later in life.	topic_ll
77486	2	356043	7	NULL	NULL	0	NULL	TL	MedicalFinding		is					transient leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Unique to newborn infants with Down syndrome is a transient leukemia (TL), also referred to as transient myeloproliferative syn- drome, that undergoes spontaneous re-mission in the majority of cases but in approximately 20% is followed by AMKL later in life.	topic_ll
77487	3	356043	7	NULL	NULL	0	NULL	TL	MedicalFinding		also referred as					transient myeloproliferative syn- drome	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Unique to newborn infants with Down syndrome is a transient leukemia (TL), also referred to as transient myeloproliferative syn- drome, that undergoes spontaneous re-mission in the majority of cases but in approximately 20% is followed by AMKL later in life.	topic_ll
77488	4	356043	7	NULL	NULL	NULL	NULL	TL	MedicalFinding		undergoes					 AMKL	MedicalFinding	spontaneous re-mission to form			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Unique to newborn infants with Down syndrome is a transient leukemia (TL), also referred to as transient myeloproliferative syn- drome, that undergoes spontaneous re-mission in the majority of cases but in approximately 20% is followed by AMKL later in life.	topic_ll
77489	5	356043	7	NULL	NULL	0	NULL	statement 4	Process		follows					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Unique to newborn infants with Down syndrome is a transient leukemia (TL), also referred to as transient myeloproliferative syn- drome, that undergoes spontaneous re-mission in the majority of cases but in approximately 20% is followed by AMKL later in life.	topic_ll
77490	1	356044	7	NULL	NULL	NULL	NULL	GATA1	GP	mutations of 	specific for					AMKL	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Recently mutations of the gene encoding the hematopoietic tran- scription factor GATA1 were shown to be specific for AMKL of Down syndrome.	topic_ll
77491	2	356044	7	NULL	NULL	0	NULL	statement 1	Process		occur in					Down syndrome	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Recently mutations of the gene encoding the hematopoietic tran- scription factor GATA1 were shown to be specific for AMKL of Down syndrome.	topic_ll
77492	3	356044	7	NULL	NULL	0	NULL	GATA1	GP		is a type of					hematopoietic tran- scription factor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Recently mutations of the gene encoding the hematopoietic tran- scription factor GATA1 were shown to be specific for AMKL of Down syndrome.	topic_ll
77493	1	356045	7	NULL	NULL	0	NULL	 GATA1 	GP	mutations of	present in					TL	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	we hypothesized that GATA1 mutations are present in TL of Down syndrome	topic_ll
77494	2	356045	7	NULL	NULL	0	NULL	statement 1	Process		occur in					Down syndrome	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	we hypothesized that GATA1 mutations are present in TL of Down syndrome	topic_ll
77495	1	356046	7	NULL	NULL	NULL	NULL	GATA1 function	Process	lack of	result in					megakaryocytes	Cell	accumulation of abnormally differentiated			NULL	hematopoietic cells	NULL	NULL	NULL	NULL	NULL	NULL	Lack of GATA1 function in hematopoietic cells had previously been shown to result in the accumulation of abnormally differentiated megakaryocytes and thrombocytopenia without leukemic transformation.	topic_ll
77496	2	356046	7	NULL	NULL	0	NULL	GATA1 function	Process	lack of	result in					thrombocytopenia	MedicalFinding				NULL	hematopoietic cells	0	NULL	NULL	NULL	NULL	NULL	Lack of GATA1 function in hematopoietic cells had previously been shown to result in the accumulation of abnormally differentiated megakaryocytes and thrombocytopenia without leukemic transformation.	topic_ll
77497	3	356046	7	NULL	NULL	0	NULL	statement 2	Process		occur without					leukemic transformation	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Lack of GATA1 function in hematopoietic cells had previously been shown to result in the accumulation of abnormally differentiated megakaryocytes and thrombocytopenia without leukemic transformation.	topic_ll
77035	1	356048	5	NULL	NULL	0	NULL	ICAM-1	GP		is					inter-cellular adhesion molecule-1	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Decreased levels of the soluble (s) inter-cellular adhesion molecule-1 (ICAM-1), as found in schizophrenia, also represent an under-activation of the type-1 immune system (Schwarz et al., 2000).	topic_sch
77036	2	356048	5	NULL	NULL	0	NULL	ICAM-1	GP	level of;;soluble	decreased in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Decreased levels of the soluble (s) inter-cellular adhesion molecule-1 (ICAM-1), as found in schizophrenia, also represent an under-activation of the type-1 immune system (Schwarz et al., 2000).	topic_sch
77037	3	356048	5	NULL	NULL	NULL	NULL	ICAM-1	GP	decreased level of;;soluble	represent					type-1 immune system	OrganismPart	under-activation of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased levels of the soluble (s) inter-cellular adhesion molecule-1 (ICAM-1), as found in schizophrenia, also represent an under-activation of the type-1 immune system (Schwarz et al., 2000).	topic_sch
77038	1	356049	5	NULL	NULL	0	NULL	p55	GP		is a type of					TNF-receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Decreased levels of the soluble TNF-receptor p55 – mostly decreased when TNF-" is decreased – were observed, too (Haack et al., 1999).	topic_sch
77039	2	356049	5	NULL	NULL	0	NULL	TNF	GP	decrease in	decreases					p55	GP	level of;;soluble			NULL		0	NULL	NULL	NULL	NULL	NULL	Decreased levels of the soluble TNF-receptor p55 – mostly decreased when TNF-" is decreased – were observed, too (Haack et al., 1999).	topic_sch
77040	1	356050	5	NULL	NULL	0	NULL	antipsychotic medication	Chemical		is a type of					confounding factor	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this meta-analysis support the view, that antipsychotic medication is a confounding factor in the analysis of the immune system in schizophrenia, upregulating type-1 immune markers.	topic_sch
77041	2	356050	5	NULL	NULL	0	NULL	statement 1	Process		in analysis of					immune system	OrganismPart	schizophrenic			NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this meta-analysis support the view, that antipsychotic medication is a confounding factor in the analysis of the immune system in schizophrenia, upregulating type-1 immune markers.	topic_sch
77042	3	356050	5	NULL	NULL	0	NULL	antipsychotic medication	Chemical		upregulates					type-1 immune markers	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this meta-analysis support the view, that antipsychotic medication is a confounding factor in the analysis of the immune system in schizophrenia, upregulating type-1 immune markers.	topic_sch
77055	1	356052	5	NULL	NULL	0	NULL	type-2 immune response	Process		is activated in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, several other signs of activation of the type-2 immune response are described in schizophrenia, including the increased Th2 type of lymphocytes in the blood (Sperner- Unterweger et al., 1999b), the increased production of Immunoglobulin E (IgE) and an increase of IL-10 serum levels (Schwarz et al., 2001; van Kammen et al., 1997).	topic_sch
77056	2	356052	5	NULL	NULL	0	NULL	Th2 lymphocytes	Cell		is present in					blood	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, several other signs of activation of the type-2 immune response are described in schizophrenia, including the increased Th2 type of lymphocytes in the blood (Sperner- Unterweger et al., 1999b), the increased production of Immunoglobulin E (IgE) and an increase of IL-10 serum levels (Schwarz et al., 2001; van Kammen et al., 1997).	topic_sch
77057	3	356052	5	NULL	NULL	0	NULL	statement 1	Process		is increased in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, several other signs of activation of the type-2 immune response are described in schizophrenia, including the increased Th2 type of lymphocytes in the blood (Sperner- Unterweger et al., 1999b), the increased production of Immunoglobulin E (IgE) and an increase of IL-10 serum levels (Schwarz et al., 2001; van Kammen et al., 1997).	topic_sch
77058	4	356052	5	NULL	NULL	0	NULL	IgE	GP		is					Immunoglobulin E	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, several other signs of activation of the type-2 immune response are described in schizophrenia, including the increased Th2 type of lymphocytes in the blood (Sperner- Unterweger et al., 1999b), the increased production of Immunoglobulin E (IgE) and an increase of IL-10 serum levels (Schwarz et al., 2001; van Kammen et al., 1997).	topic_sch
77059	5	356052	5	NULL	NULL	0	NULL	IgE	GP	production of	is increased in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, several other signs of activation of the type-2 immune response are described in schizophrenia, including the increased Th2 type of lymphocytes in the blood (Sperner- Unterweger et al., 1999b), the increased production of Immunoglobulin E (IgE) and an increase of IL-10 serum levels (Schwarz et al., 2001; van Kammen et al., 1997).	topic_sch
77060	6	356052	5	NULL	NULL	0	NULL	IL-10	GP	levels of;;serum	is increased in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover, several other signs of activation of the type-2 immune response are described in schizophrenia, including the increased Th2 type of lymphocytes in the blood (Sperner- Unterweger et al., 1999b), the increased production of Immunoglobulin E (IgE) and an increase of IL-10 serum levels (Schwarz et al., 2001; van Kammen et al., 1997).	topic_sch
77061	1	356053	5	NULL	NULL	0	NULL	IL-4	GP	levels of	is increased in					schizophrenic patients	GroupOfPeople	juvenile			NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of IL-4 in the CSF of juvenile schizophrenic patients have been reported (Mittleman et al., 1997), which indicates that the increased type-2 response in schizophrenia is not only a phenomenon of the peripheral immune response.	topic_sch
77062	2	356053	5	NULL	NULL	0	NULL	type-2 response	Process		is increased in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of IL-4 in the CSF of juvenile schizophrenic patients have been reported (Mittleman et al., 1997), which indicates that the increased type-2 response in schizophrenia is not only a phenomenon of the peripheral immune response.	topic_sch
77063	3	356053	5	NULL	NULL	0	NULL	statement 2	Process		is a type of					peripheral immune response	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of IL-4 in the CSF of juvenile schizophrenic patients have been reported (Mittleman et al., 1997), which indicates that the increased type-2 response in schizophrenia is not only a phenomenon of the peripheral immune response.	topic_sch
77498	1	356054	7	NULL	NULL	0	NULL	GSK3	GP		therapeutic target in		potential			bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Preclinical studies have suggested that glycogen synthase kinase-3 (GSK3) is a potential therapeutic target in bipolar disorder, but evidence of abnormal GSK3 in human bipolar disorder and its response to treatment is still lacking.	topic_bd
77499	2	356054	7	NULL	NULL	0	NULL	GSK3	GP		is					glycogen synthase kinase-3	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Preclinical studies have suggested that glycogen synthase kinase-3 (GSK3) is a potential therapeutic target in bipolar disorder, but evidence of abnormal GSK3 in human bipolar disorder and its response to treatment is still lacking.	topic_bd
77500	1	356055	7	NULL	NULL	0	NULL	CCNH	GP	genetic variants in	associated with		strongly			CLL 	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	After adjustment for multiple testing, strong associations were identified between CLL risk and genetic variants in CCNH, APAF1, IL16, CASP8, NOS2A, and CCR7. 	topic_ll
77501	2	356055	7	NULL	NULL	0	NULL	APAF1	GP	genetic variants in	associated with		strongly			CLL	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	After adjustment for multiple testing, strong associations were identified between CLL risk and genetic variants in CCNH, APAF1, IL16, CASP8, NOS2A, and CCR7. 	topic_ll
77502	3	356055	7	NULL	NULL	0	NULL	IL16	GP	genetic variants in	associated with		strongly			CLL	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	After adjustment for multiple testing, strong associations were identified between CLL risk and genetic variants in CCNH, APAF1, IL16, CASP8, NOS2A, and CCR7. 	topic_ll
77503	4	356055	7	NULL	NULL	0	NULL	CASP8	GP	genetic variants in	associated with		strongly			CLL	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	After adjustment for multiple testing, strong associations were identified between CLL risk and genetic variants in CCNH, APAF1, IL16, CASP8, NOS2A, and CCR7. 	topic_ll
77504	5	356055	7	NULL	NULL	0	NULL	NOS2A	GP	genetic variants in	associated with		strongly			CLL	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	After adjustment for multiple testing, strong associations were identified between CLL risk and genetic variants in CCNH, APAF1, IL16, CASP8, NOS2A, and CCR7. 	topic_ll
77505	6	356055	7	NULL	NULL	0	NULL	CCR7	GP	genetic variants in	associated with		strongly			CLL	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	After adjustment for multiple testing, strong associations were identified between CLL risk and genetic variants in CCNH, APAF1, IL16, CASP8, NOS2A, and CCR7. 	topic_ll
77506	1	356056	7	NULL	NULL	NULL	NULL	CCNH gene	GP	humans	encode					Cyclin-H protein	GP	humans			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclin-H is a protein that in humans is encoded by the CCNH gene.	topic_ll
77507	1	356057	7	NULL	NULL	0	NULL	PI3 kinase	GP		promotes					CLL B cells	Cell	survival of			NULL		0	NULL	NULL	NULL	NULL	NULL	PI3 kinase promotes survival of chronic lymphocytic leukemia (CLL) B cells by preventing caspase-8 activation.	topic_ll
77508	2	356057	7	NULL	NULL	0	NULL	statement 1	Process		prevent					caspase-8	GP	activation of			NULL		0	NULL	NULL	NULL	NULL	NULL	PI3 kinase promotes survival of chronic lymphocytic leukemia (CLL) B cells by preventing caspase-8 activation.	topic_ll
77509	3	356057	7	NULL	NULL	0	NULL	CLL	MedicalFinding		is					chronic lymphocytic leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	PI3 kinase promotes survival of chronic lymphocytic leukemia (CLL) B cells by preventing caspase-8 activation.	topic_ll
77510	1	356058	7	NULL	NULL	0	NULL	Fas-L	GP		ligates					Fas molecule	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Ligation of the cell-surface Fas molecule by its ligand (Fas-L) or agonistic anti-Fas monoclonal antibodies results in the cleavage and activation of the cysteine protease procaspase 8 followed by the activation of procaspase 3 and by apoptosis.	topic_ll
77511	2	356058	7	NULL	NULL	0	NULL	anti-Fas monoclonal antibodies	GP		ligates					Fas molecule	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Ligation of the cell-surface Fas molecule by its ligand (Fas-L) or agonistic anti-Fas monoclonal antibodies results in the cleavage and activation of the cysteine protease procaspase 8 followed by the activation of procaspase 3 and by apoptosis.	topic_ll
77512	3	356058	7	NULL	NULL	NULL	NULL	statement 1	Process		results in					procaspase 8	GP	cleavage of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ligation of the cell-surface Fas molecule by its ligand (Fas-L) or agonistic anti-Fas monoclonal antibodies results in the cleavage and activation of the cysteine protease procaspase 8 followed by the activation of procaspase 3 and by apoptosis.	topic_ll
77513	4	356058	7	NULL	NULL	NULL	NULL	statement 2	Process		results in					procaspase 8	GP	cleavage of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ligation of the cell-surface Fas molecule by its ligand (Fas-L) or agonistic anti-Fas monoclonal antibodies results in the cleavage and activation of the cysteine protease procaspase 8 followed by the activation of procaspase 3 and by apoptosis.	topic_ll
77514	5	356058	7	NULL	NULL	0	NULL	statement 1	Process		results in					procaspase 8	GP	activation of			NULL		0	NULL	NULL	NULL	NULL	NULL	Ligation of the cell-surface Fas molecule by its ligand (Fas-L) or agonistic anti-Fas monoclonal antibodies results in the cleavage and activation of the cysteine protease procaspase 8 followed by the activation of procaspase 3 and by apoptosis.	topic_ll
77515	6	356058	7	NULL	NULL	0	NULL	statement 2	Process		results in					procaspase 8	GP	activation of			NULL		0	NULL	NULL	NULL	NULL	NULL	Ligation of the cell-surface Fas molecule by its ligand (Fas-L) or agonistic anti-Fas monoclonal antibodies results in the cleavage and activation of the cysteine protease procaspase 8 followed by the activation of procaspase 3 and by apoptosis.	topic_ll
77516	7	356058	7	NULL	NULL	0	NULL	statement 3	Process		occur with					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Ligation of the cell-surface Fas molecule by its ligand (Fas-L) or agonistic anti-Fas monoclonal antibodies results in the cleavage and activation of the cysteine protease procaspase 8 followed by the activation of procaspase 3 and by apoptosis.	topic_ll
77517	8	356058	7	NULL	NULL	0	NULL	statement 4	Process		occur with					statement 6	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Ligation of the cell-surface Fas molecule by its ligand (Fas-L) or agonistic anti-Fas monoclonal antibodies results in the cleavage and activation of the cysteine protease procaspase 8 followed by the activation of procaspase 3 and by apoptosis.	topic_ll
77518	9	356058	7	NULL	NULL	0	NULL	statement 7	Process		followed by					procaspase 3	GP	activation of			NULL		0	NULL	NULL	NULL	NULL	NULL	Ligation of the cell-surface Fas molecule by its ligand (Fas-L) or agonistic anti-Fas monoclonal antibodies results in the cleavage and activation of the cysteine protease procaspase 8 followed by the activation of procaspase 3 and by apoptosis.	topic_ll
77519	10	356058	7	NULL	NULL	0	NULL	statement 8	Process		followed by					procaspase 3	GP	activation of			NULL		0	NULL	NULL	NULL	NULL	NULL	Ligation of the cell-surface Fas molecule by its ligand (Fas-L) or agonistic anti-Fas monoclonal antibodies results in the cleavage and activation of the cysteine protease procaspase 8 followed by the activation of procaspase 3 and by apoptosis.	topic_ll
77520	11	356058	7	NULL	NULL	0	NULL	statement 7	Process		followed by					apoptosis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Ligation of the cell-surface Fas molecule by its ligand (Fas-L) or agonistic anti-Fas monoclonal antibodies results in the cleavage and activation of the cysteine protease procaspase 8 followed by the activation of procaspase 3 and by apoptosis.	topic_ll
77521	12	356058	7	NULL	NULL	0	NULL	statement 8	Process		followed by					apoptosis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Ligation of the cell-surface Fas molecule by its ligand (Fas-L) or agonistic anti-Fas monoclonal antibodies results in the cleavage and activation of the cysteine protease procaspase 8 followed by the activation of procaspase 3 and by apoptosis.	topic_ll
77522	13	356058	7	NULL	NULL	0	NULL	Fas molecule 	GP		is a type of					cell-surface molecule	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Ligation of the cell-surface Fas molecule by its ligand (Fas-L) or agonistic anti-Fas monoclonal antibodies results in the cleavage and activation of the cysteine protease procaspase 8 followed by the activation of procaspase 3 and by apoptosis.	topic_ll
77523	14	356058	7	NULL	NULL	0	NULL	procaspase 8	GP		is a type of					cysteine protease	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Ligation of the cell-surface Fas molecule by its ligand (Fas-L) or agonistic anti-Fas monoclonal antibodies results in the cleavage and activation of the cysteine protease procaspase 8 followed by the activation of procaspase 3 and by apoptosis.	topic_ll
77524	1	356059	7	NULL	NULL	0	NULL	cytotoxic drugs	Chemical		induce					Fas-L	GP	expression of			NULL	leukemia cell lines	0	NULL	NULL	NULL	NULL	NULL	In some leukemia cell lines, cytotoxic drugs induce expression of Fas-L, which may contribute to cell killing through the ligation of Fas. These data suggest that the Fas/Fas-L signaling system does not play a major role in the induction of apoptosis in B-CLL cells treated with cytotoxic drugs or radiation. However, Fas-independent activation of caspase 8 may play a crucial role in the regulation of apoptosis in these cells.	topic_ll
77525	2	356059	7	NULL	NULL	NULL	NULL	statement 1	Process		contribute to		may			cell 	Cell	killing of			NULL	leukemia cell lines	NULL	NULL	NULL	NULL	NULL	NULL	In some leukemia cell lines, cytotoxic drugs induce expression of Fas-L, which may contribute to cell killing through the ligation of Fas. These data suggest that the Fas/Fas-L signaling system does not play a major role in the induction of apoptosis in B-CLL cells treated with cytotoxic drugs or radiation. However, Fas-independent activation of caspase 8 may play a crucial role in the regulation of apoptosis in these cells.	topic_ll
77526	3	356059	7	NULL	NULL	NULL	NULL	statement 2	Process		occur through					Fas	GP	ligation of			NULL	leukemia cell lines	NULL	NULL	NULL	NULL	NULL	NULL	In some leukemia cell lines, cytotoxic drugs induce expression of Fas-L, which may contribute to cell killing through the ligation of Fas. These data suggest that the Fas/Fas-L signaling system does not play a major role in the induction of apoptosis in B-CLL cells treated with cytotoxic drugs or radiation. However, Fas-independent activation of caspase 8 may play a crucial role in the regulation of apoptosis in these cells.	topic_ll
77527	4	356059	7	NULL	NULL	0	NULL	Fas/Fas-L signaling	Process		does not play					apoptosis	Process	major role in induction of			NULL		0	NULL	NULL	NULL	NULL	NULL	In some leukemia cell lines, cytotoxic drugs induce expression of Fas-L, which may contribute to cell killing through the ligation of Fas. These data suggest that the Fas/Fas-L signaling system does not play a major role in the induction of apoptosis in B-CLL cells treated with cytotoxic drugs or radiation. However, Fas-independent activation of caspase 8 may play a crucial role in the regulation of apoptosis in these cells.	topic_ll
77528	5	356059	7	NULL	NULL	0	NULL	B-CLL cells	Cell		treated with					cytotoxic drugs	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	In some leukemia cell lines, cytotoxic drugs induce expression of Fas-L, which may contribute to cell killing through the ligation of Fas. These data suggest that the Fas/Fas-L signaling system does not play a major role in the induction of apoptosis in B-CLL cells treated with cytotoxic drugs or radiation. However, Fas-independent activation of caspase 8 may play a crucial role in the regulation of apoptosis in these cells.	topic_ll
77529	6	356059	7	NULL	NULL	0	NULL	B-CLL cells	Cell		treated with					radiation	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	In some leukemia cell lines, cytotoxic drugs induce expression of Fas-L, which may contribute to cell killing through the ligation of Fas. These data suggest that the Fas/Fas-L signaling system does not play a major role in the induction of apoptosis in B-CLL cells treated with cytotoxic drugs or radiation. However, Fas-independent activation of caspase 8 may play a crucial role in the regulation of apoptosis in these cells.	topic_ll
77530	7	356059	7	NULL	NULL	0	NULL	statement 4	Process		occur in					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	In some leukemia cell lines, cytotoxic drugs induce expression of Fas-L, which may contribute to cell killing through the ligation of Fas. These data suggest that the Fas/Fas-L signaling system does not play a major role in the induction of apoptosis in B-CLL cells treated with cytotoxic drugs or radiation. However, Fas-independent activation of caspase 8 may play a crucial role in the regulation of apoptosis in these cells.	topic_ll
77531	8	356059	7	NULL	NULL	0	NULL	statement 4	Process		occur in					statement 6	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	In some leukemia cell lines, cytotoxic drugs induce expression of Fas-L, which may contribute to cell killing through the ligation of Fas. These data suggest that the Fas/Fas-L signaling system does not play a major role in the induction of apoptosis in B-CLL cells treated with cytotoxic drugs or radiation. However, Fas-independent activation of caspase 8 may play a crucial role in the regulation of apoptosis in these cells.	topic_ll
77532	9	356059	7	NULL	NULL	0	NULL	statement 7	Process		is an alternative to					statement 8	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	In some leukemia cell lines, cytotoxic drugs induce expression of Fas-L, which may contribute to cell killing through the ligation of Fas. These data suggest that the Fas/Fas-L signaling system does not play a major role in the induction of apoptosis in B-CLL cells treated with cytotoxic drugs or radiation. However, Fas-independent activation of caspase 8 may play a crucial role in the regulation of apoptosis in these cells.	topic_ll
77533	10	356059	7	NULL	NULL	NULL	NULL	caspase 8	GP	activation of	is independent of					Fas	GP				NULL	leukemia cell lines	NULL	NULL	NULL	NULL	NULL	NULL	In some leukemia cell lines, cytotoxic drugs induce expression of Fas-L, which may contribute to cell killing through the ligation of Fas. These data suggest that the Fas/Fas-L signaling system does not play a major role in the induction of apoptosis in B-CLL cells treated with cytotoxic drugs or radiation. However, Fas-independent activation of caspase 8 may play a crucial role in the regulation of apoptosis in these cells.	topic_ll
77534	11	356059	7	NULL	NULL	NULL	NULL	statement 10	Process		play crucial role in		may			apoptosis	Process	regulation of			NULL	leukemia cell lines	NULL	NULL	NULL	NULL	NULL	NULL	In some leukemia cell lines, cytotoxic drugs induce expression of Fas-L, which may contribute to cell killing through the ligation of Fas. These data suggest that the Fas/Fas-L signaling system does not play a major role in the induction of apoptosis in B-CLL cells treated with cytotoxic drugs or radiation. However, Fas-independent activation of caspase 8 may play a crucial role in the regulation of apoptosis in these cells.	topic_ll
77535	1	356061	7	NULL	NULL	0	NULL	CLL risk loci	Chromosome		identified at					6p25.3 (IRF4)	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	Six previously unreported CLL risk loci were identified at 6p25.3 (IRF4), 19q13.32 (PRKD2), 2q37.1 (SP140), 2q13, 11q24.1, and 15q23 for which there was statistically significant evidence for an association on a genome-wide basis (i.e. p<10–7).	topic_ll
77536	2	356061	7	NULL	NULL	0	NULL	CLL risk loci	Chromosome		identified at					19q13.32 (PRKD2)	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	Six previously unreported CLL risk loci were identified at 6p25.3 (IRF4), 19q13.32 (PRKD2), 2q37.1 (SP140), 2q13, 11q24.1, and 15q23 for which there was statistically significant evidence for an association on a genome-wide basis (i.e. p<10–7).	topic_ll
77537	3	356061	7	NULL	NULL	0	NULL	CLL risk loci	Chromosome		identified at					2q37.1 (SP140)	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	Six previously unreported CLL risk loci were identified at 6p25.3 (IRF4), 19q13.32 (PRKD2), 2q37.1 (SP140), 2q13, 11q24.1, and 15q23 for which there was statistically significant evidence for an association on a genome-wide basis (i.e. p<10–7).	topic_ll
77538	4	356061	7	NULL	NULL	0	NULL	CLL risk loci 	Chromosome		identified at					2q13	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	Six previously unreported CLL risk loci were identified at 6p25.3 (IRF4), 19q13.32 (PRKD2), 2q37.1 (SP140), 2q13, 11q24.1, and 15q23 for which there was statistically significant evidence for an association on a genome-wide basis (i.e. p<10–7).	topic_ll
77539	5	356061	7	NULL	NULL	0	NULL	CLL risk loci	Chromosome		identified at					11q24.1	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	Six previously unreported CLL risk loci were identified at 6p25.3 (IRF4), 19q13.32 (PRKD2), 2q37.1 (SP140), 2q13, 11q24.1, and 15q23 for which there was statistically significant evidence for an association on a genome-wide basis (i.e. p<10–7).	topic_ll
77540	6	356061	7	NULL	NULL	NULL	NULL	CLL risk loci	Chromosome		identified at					15q23	Chromosome				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Six previously unreported CLL risk loci were identified at 6p25.3 (IRF4), 19q13.32 (PRKD2), 2q37.1 (SP140), 2q13, 11q24.1, and 15q23 for which there was statistically significant evidence for an association on a genome-wide basis (i.e. p<10–7).	topic_ll
77541	1	356062	7	NULL	NULL	0	NULL	SP140	GP		lymphoid-restricted homolog of					SP100	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	SP140 is the lymphoid-restricted homolog of SP100, expressed in all mature B cells and plasma cell lines, as well as some T cells. SP100 is a major mediator of EBNA-LP (Epstein- Barr virus (EBV) encoded nuclear antigen leader protein), whose co-activation is important for establishing latent viral infections and EBV-mediated B-cell immortalization. A significant dose relationship between rs13397985 genotype and SP140 expression in lymphocytes was demonstrable, with risk alleles being associated with reduced levels of mRNA. SP140 expression has been implicated in innate response to immunodeficiency virus type 1; hence, although speculative, it is possible that genetic variation in SP140 influences the risk of developing CLL through differing response to antigenic challenge.	topic_ll
77542	2	356062	7	NULL	NULL	0	NULL	SP140	GP		expressed in					mature B cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	SP140 is the lymphoid-restricted homolog of SP100, expressed in all mature B cells and plasma cell lines, as well as some T cells. SP100 is a major mediator of EBNA-LP (Epstein- Barr virus (EBV) encoded nuclear antigen leader protein), whose co-activation is important for establishing latent viral infections and EBV-mediated B-cell immortalization. A significant dose relationship between rs13397985 genotype and SP140 expression in lymphocytes was demonstrable, with risk alleles being associated with reduced levels of mRNA. SP140 expression has been implicated in innate response to immunodeficiency virus type 1; hence, although speculative, it is possible that genetic variation in SP140 influences the risk of developing CLL through differing response to antigenic challenge.	topic_ll
77543	3	356062	7	NULL	NULL	0	NULL	SP140	GP		expressed in					plasma cell lines	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	SP140 is the lymphoid-restricted homolog of SP100, expressed in all mature B cells and plasma cell lines, as well as some T cells. SP100 is a major mediator of EBNA-LP (Epstein- Barr virus (EBV) encoded nuclear antigen leader protein), whose co-activation is important for establishing latent viral infections and EBV-mediated B-cell immortalization. A significant dose relationship between rs13397985 genotype and SP140 expression in lymphocytes was demonstrable, with risk alleles being associated with reduced levels of mRNA. SP140 expression has been implicated in innate response to immunodeficiency virus type 1; hence, although speculative, it is possible that genetic variation in SP140 influences the risk of developing CLL through differing response to antigenic challenge.	topic_ll
77544	4	356062	7	NULL	NULL	0	NULL	SP140	GP		expressed in					T cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	SP140 is the lymphoid-restricted homolog of SP100, expressed in all mature B cells and plasma cell lines, as well as some T cells. SP100 is a major mediator of EBNA-LP (Epstein- Barr virus (EBV) encoded nuclear antigen leader protein), whose co-activation is important for establishing latent viral infections and EBV-mediated B-cell immortalization. A significant dose relationship between rs13397985 genotype and SP140 expression in lymphocytes was demonstrable, with risk alleles being associated with reduced levels of mRNA. SP140 expression has been implicated in innate response to immunodeficiency virus type 1; hence, although speculative, it is possible that genetic variation in SP140 influences the risk of developing CLL through differing response to antigenic challenge.	topic_ll
77545	5	356062	7	NULL	NULL	0	NULL	SP100	GP		mediator of		major			EBNA-LP	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	SP140 is the lymphoid-restricted homolog of SP100, expressed in all mature B cells and plasma cell lines, as well as some T cells. SP100 is a major mediator of EBNA-LP (Epstein- Barr virus (EBV) encoded nuclear antigen leader protein), whose co-activation is important for establishing latent viral infections and EBV-mediated B-cell immortalization. A significant dose relationship between rs13397985 genotype and SP140 expression in lymphocytes was demonstrable, with risk alleles being associated with reduced levels of mRNA. SP140 expression has been implicated in innate response to immunodeficiency virus type 1; hence, although speculative, it is possible that genetic variation in SP140 influences the risk of developing CLL through differing response to antigenic challenge.	topic_ll
77546	6	356062	7	NULL	NULL	0	NULL	EBNA-LP	GP		is					Epstein- Barr virus encoded nuclear antigen leader protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	SP140 is the lymphoid-restricted homolog of SP100, expressed in all mature B cells and plasma cell lines, as well as some T cells. SP100 is a major mediator of EBNA-LP (Epstein- Barr virus (EBV) encoded nuclear antigen leader protein), whose co-activation is important for establishing latent viral infections and EBV-mediated B-cell immortalization. A significant dose relationship between rs13397985 genotype and SP140 expression in lymphocytes was demonstrable, with risk alleles being associated with reduced levels of mRNA. SP140 expression has been implicated in innate response to immunodeficiency virus type 1; hence, although speculative, it is possible that genetic variation in SP140 influences the risk of developing CLL through differing response to antigenic challenge.	topic_ll
77547	7	356062	7	NULL	NULL	0	NULL	EBNA-LP	GP	coactivation of	is important for					latent viral infections	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	SP140 is the lymphoid-restricted homolog of SP100, expressed in all mature B cells and plasma cell lines, as well as some T cells. SP100 is a major mediator of EBNA-LP (Epstein- Barr virus (EBV) encoded nuclear antigen leader protein), whose co-activation is important for establishing latent viral infections and EBV-mediated B-cell immortalization. A significant dose relationship between rs13397985 genotype and SP140 expression in lymphocytes was demonstrable, with risk alleles being associated with reduced levels of mRNA. SP140 expression has been implicated in innate response to immunodeficiency virus type 1; hence, although speculative, it is possible that genetic variation in SP140 influences the risk of developing CLL through differing response to antigenic challenge.	topic_ll
77548	8	356062	7	NULL	NULL	0	NULL	EBV	Organism		mediates					B-cell immortalization	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	SP140 is the lymphoid-restricted homolog of SP100, expressed in all mature B cells and plasma cell lines, as well as some T cells. SP100 is a major mediator of EBNA-LP (Epstein- Barr virus (EBV) encoded nuclear antigen leader protein), whose co-activation is important for establishing latent viral infections and EBV-mediated B-cell immortalization. A significant dose relationship between rs13397985 genotype and SP140 expression in lymphocytes was demonstrable, with risk alleles being associated with reduced levels of mRNA. SP140 expression has been implicated in innate response to immunodeficiency virus type 1; hence, although speculative, it is possible that genetic variation in SP140 influences the risk of developing CLL through differing response to antigenic challenge.	topic_ll
77549	9	356062	7	NULL	NULL	0	NULL	EBNA-LP	GP	coactivation of	is important for					statement 8	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	SP140 is the lymphoid-restricted homolog of SP100, expressed in all mature B cells and plasma cell lines, as well as some T cells. SP100 is a major mediator of EBNA-LP (Epstein- Barr virus (EBV) encoded nuclear antigen leader protein), whose co-activation is important for establishing latent viral infections and EBV-mediated B-cell immortalization. A significant dose relationship between rs13397985 genotype and SP140 expression in lymphocytes was demonstrable, with risk alleles being associated with reduced levels of mRNA. SP140 expression has been implicated in innate response to immunodeficiency virus type 1; hence, although speculative, it is possible that genetic variation in SP140 influences the risk of developing CLL through differing response to antigenic challenge.	topic_ll
77550	10	356062	7	NULL	NULL	NULL	NULL	rs13397985 genotype	GP		exist in 					SP140	GP	relationship with expression of			NULL	lymphocytes	NULL	NULL	NULL	NULL	NULL	NULL	SP140 is the lymphoid-restricted homolog of SP100, expressed in all mature B cells and plasma cell lines, as well as some T cells. SP100 is a major mediator of EBNA-LP (Epstein- Barr virus (EBV) encoded nuclear antigen leader protein), whose co-activation is important for establishing latent viral infections and EBV-mediated B-cell immortalization. A significant dose relationship between rs13397985 genotype and SP140 expression in lymphocytes was demonstrable, with risk alleles being associated with reduced levels of mRNA. SP140 expression has been implicated in innate response to immunodeficiency virus type 1; hence, although speculative, it is possible that genetic variation in SP140 influences the risk of developing CLL through differing response to antigenic challenge.	topic_ll
77551	11	356062	7	NULL	NULL	0	NULL	SP140 	GP	expression of	has been implicated in					 immunodeficiency virus type 1	Organism	innate response to			NULL		0	NULL	NULL	NULL	NULL	NULL	SP140 is the lymphoid-restricted homolog of SP100, expressed in all mature B cells and plasma cell lines, as well as some T cells. SP100 is a major mediator of EBNA-LP (Epstein- Barr virus (EBV) encoded nuclear antigen leader protein), whose co-activation is important for establishing latent viral infections and EBV-mediated B-cell immortalization. A significant dose relationship between rs13397985 genotype and SP140 expression in lymphocytes was demonstrable, with risk alleles being associated with reduced levels of mRNA. SP140 expression has been implicated in innate response to immunodeficiency virus type 1; hence, although speculative, it is possible that genetic variation in SP140 influences the risk of developing CLL through differing response to antigenic challenge.	topic_ll
77552	12	356062	7	NULL	NULL	NULL	NULL	SP140	GP	genetic variation in	influence					CLL	MedicalFinding	risk of developing			NULL		NULL	NULL	NULL	NULL	NULL	NULL	SP140 is the lymphoid-restricted homolog of SP100, expressed in all mature B cells and plasma cell lines, as well as some T cells. SP100 is a major mediator of EBNA-LP (Epstein- Barr virus (EBV) encoded nuclear antigen leader protein), whose co-activation is important for establishing latent viral infections and EBV-mediated B-cell immortalization. A significant dose relationship between rs13397985 genotype and SP140 expression in lymphocytes was demonstrable, with risk alleles being associated with reduced levels of mRNA. SP140 expression has been implicated in innate response to immunodeficiency virus type 1; hence, although speculative, it is possible that genetic variation in SP140 influences the risk of developing CLL through differing response to antigenic challenge.	topic_ll
77553	13	356062	7	NULL	NULL	0	NULL	statement 12	Process		occur through					antigenic challenge	Process	response to			NULL		0	NULL	NULL	NULL	NULL	NULL	SP140 is the lymphoid-restricted homolog of SP100, expressed in all mature B cells and plasma cell lines, as well as some T cells. SP100 is a major mediator of EBNA-LP (Epstein- Barr virus (EBV) encoded nuclear antigen leader protein), whose co-activation is important for establishing latent viral infections and EBV-mediated B-cell immortalization. A significant dose relationship between rs13397985 genotype and SP140 expression in lymphocytes was demonstrable, with risk alleles being associated with reduced levels of mRNA. SP140 expression has been implicated in innate response to immunodeficiency virus type 1; hence, although speculative, it is possible that genetic variation in SP140 influences the risk of developing CLL through differing response to antigenic challenge.	topic_ll
77554	1	356063	7	NULL	NULL	0	NULL	MBL	MedicalFinding		develops into					CLL	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Intriguingly this assertion is supported by the observation that CLL-phenotype B cells (CD5+, CD23+, CD20low, sIgMlow) of monoclonal B-cell lymphocytosis (MBL) are detectable in ~ 3% of adults in the general population26 and that they are essentially indistinguishable from CLL B cells in terms of chromosomal abnormalities and IgVH mutation status. The recent report that MBL develops into CLL at a rate of 1.1% per year provides direct evidence that MBL is a precursor lesion for CLL. 	topic_ll
77555	2	356063	7	NULL	NULL	0	NULL	MBL	MedicalFinding		is a precursor lesion for					CLL	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Intriguingly this assertion is supported by the observation that CLL-phenotype B cells (CD5+, CD23+, CD20low, sIgMlow) of monoclonal B-cell lymphocytosis (MBL) are detectable in ~ 3% of adults in the general population26 and that they are essentially indistinguishable from CLL B cells in terms of chromosomal abnormalities and IgVH mutation status. The recent report that MBL develops into CLL at a rate of 1.1% per year provides direct evidence that MBL is a precursor lesion for CLL. 	topic_ll
77556	3	356063	7	NULL	NULL	0	NULL	MBL	MedicalFinding		is					monoclonal B-cell lymphocytosis	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Intriguingly this assertion is supported by the observation that CLL-phenotype B cells (CD5+, CD23+, CD20low, sIgMlow) of monoclonal B-cell lymphocytosis (MBL) are detectable in ~ 3% of adults in the general population26 and that they are essentially indistinguishable from CLL B cells in terms of chromosomal abnormalities and IgVH mutation status. The recent report that MBL develops into CLL at a rate of 1.1% per year provides direct evidence that MBL is a precursor lesion for CLL. 	topic_ll
77557	4	356063	7	NULL	NULL	0	NULL	CLL-phenotype B cells 	Cell		indistinguishable from		essentially			CLL B cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Intriguingly this assertion is supported by the observation that CLL-phenotype B cells (CD5+, CD23+, CD20low, sIgMlow) of monoclonal B-cell lymphocytosis (MBL) are detectable in ~ 3% of adults in the general population26 and that they are essentially indistinguishable from CLL B cells in terms of chromosomal abnormalities and IgVH mutation status. The recent report that MBL develops into CLL at a rate of 1.1% per year provides direct evidence that MBL is a precursor lesion for CLL. 	topic_ll
77558	5	356063	7	NULL	NULL	0	NULL	statement 4	Process		in terms of					chromosomal abnormalities	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Intriguingly this assertion is supported by the observation that CLL-phenotype B cells (CD5+, CD23+, CD20low, sIgMlow) of monoclonal B-cell lymphocytosis (MBL) are detectable in ~ 3% of adults in the general population26 and that they are essentially indistinguishable from CLL B cells in terms of chromosomal abnormalities and IgVH mutation status. The recent report that MBL develops into CLL at a rate of 1.1% per year provides direct evidence that MBL is a precursor lesion for CLL. 	topic_ll
77559	6	356063	7	NULL	NULL	0	NULL	statement 4	Process		in terms of					IgVH mutation status	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Intriguingly this assertion is supported by the observation that CLL-phenotype B cells (CD5+, CD23+, CD20low, sIgMlow) of monoclonal B-cell lymphocytosis (MBL) are detectable in ~ 3% of adults in the general population26 and that they are essentially indistinguishable from CLL B cells in terms of chromosomal abnormalities and IgVH mutation status. The recent report that MBL develops into CLL at a rate of 1.1% per year provides direct evidence that MBL is a precursor lesion for CLL. 	topic_ll
77560	7	356063	7	NULL	NULL	0	NULL	statement 1	Process		evidence for		direct			statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Intriguingly this assertion is supported by the observation that CLL-phenotype B cells (CD5+, CD23+, CD20low, sIgMlow) of monoclonal B-cell lymphocytosis (MBL) are detectable in ~ 3% of adults in the general population26 and that they are essentially indistinguishable from CLL B cells in terms of chromosomal abnormalities and IgVH mutation status. The recent report that MBL develops into CLL at a rate of 1.1% per year provides direct evidence that MBL is a precursor lesion for CLL. 	topic_ll
77561	1	356064	7	NULL	NULL	0	NULL	IgVH	GP	mutation status of	prognostic marker in					CLL	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	IgVH mutation status is a well accepted prognostic marker in chronic lymphocytic leukemia (CLL). 	topic_ll
77562	2	356064	7	NULL	NULL	0	NULL	CLL	MedicalFinding		is					chronic lymphocytic leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	IgVH mutation status is a well accepted prognostic marker in chronic lymphocytic leukemia (CLL). 	topic_ll
77563	1	356065	7	NULL	NULL	NULL	NULL	CLL	MedicalFinding	development of	influenced by					antigenic recognition	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Evidence suggests that the development of CLL might be influenced by antigenic recognition or selection through the B-cell receptor (BCR).	topic_ll
77564	2	356065	7	NULL	NULL	NULL	NULL	CLL	MedicalFinding	development of	influenced by					antigenic selection	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Evidence suggests that the development of CLL might be influenced by antigenic recognition or selection through the B-cell receptor (BCR).	topic_ll
77565	3	356065	7	NULL	NULL	0	NULL	statement 1	Process		occur through					BCR	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence suggests that the development of CLL might be influenced by antigenic recognition or selection through the B-cell receptor (BCR).	topic_ll
77566	4	356065	7	NULL	NULL	0	NULL	statement 2	Process		occur through					BCR	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence suggests that the development of CLL might be influenced by antigenic recognition or selection through the B-cell receptor (BCR).	topic_ll
77567	5	356065	7	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence suggests that the development of CLL might be influenced by antigenic recognition or selection through the B-cell receptor (BCR).	topic_ll
77568	6	356065	7	NULL	NULL	0	NULL	BCR	GP		is					B-cell receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence suggests that the development of CLL might be influenced by antigenic recognition or selection through the B-cell receptor (BCR).	topic_ll
77569	1	356066	7	NULL	NULL	0	NULL	IGHV1-69	GP	Asymmetric usage of	characterized in					CLL	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Asymmetric usage of the immunoglobulin genes have been well characterized in CLL, with notable overrepresentation of various genes, including IGHV1-69 and IGHV4-34.	topic_ll
77570	2	356066	7	NULL	NULL	0	NULL	IGHV4-34	GP	Asymmetric usage of	characterized in					CLL	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Asymmetric usage of the immunoglobulin genes have been well characterized in CLL, with notable overrepresentation of various genes, including IGHV1-69 and IGHV4-34.	topic_ll
77571	1	356067	7	NULL	NULL	0	NULL	B cells	Cell	Preferential stimulation of	express					IGHV4-34 gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Preferential stimulation of B cells expressing the IGHV4-34 gene occurs in a number of infections, including those caused by Epstein-Barr virus (EBV) and cytomegalovirus (CMV).	topic_ll
77572	2	356067	7	NULL	NULL	0	NULL	EBV	Organism	infection of	cause					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Preferential stimulation of B cells expressing the IGHV4-34 gene occurs in a number of infections, including those caused by Epstein-Barr virus (EBV) and cytomegalovirus (CMV).	topic_ll
77573	3	356067	7	NULL	NULL	0	NULL	CMV	Organism	infection of	cause					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Preferential stimulation of B cells expressing the IGHV4-34 gene occurs in a number of infections, including those caused by Epstein-Barr virus (EBV) and cytomegalovirus (CMV).	topic_ll
77574	4	356067	7	NULL	NULL	0	NULL	EBV	Organism		is involved in					Epstein-Barr virus	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Preferential stimulation of B cells expressing the IGHV4-34 gene occurs in a number of infections, including those caused by Epstein-Barr virus (EBV) and cytomegalovirus (CMV).	topic_ll
77575	5	356067	7	NULL	NULL	0	NULL	CMV	Organism		is					cytomegalovirus	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Preferential stimulation of B cells expressing the IGHV4-34 gene occurs in a number of infections, including those caused by Epstein-Barr virus (EBV) and cytomegalovirus (CMV).	topic_ll
77576	1	356068	7	NULL	NULL	0	NULL	Resveratrol	Chemical		blocks					cancer promoting genes	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Resveratrol: This phytochemical blocks the actions of a number of a number of cancer promoting genes thereby causing cancer cells to enter into apoptosis (cell death) and is included in the treatment of all cancers.	topic_ll
77577	2	356068	7	NULL	NULL	0	NULL	cancer cells	Cell		enter into					apoptosis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Resveratrol: This phytochemical blocks the actions of a number of a number of cancer promoting genes thereby causing cancer cells to enter into apoptosis (cell death) and is included in the treatment of all cancers.	topic_ll
77578	3	356068	7	NULL	NULL	0	NULL	statement 1	Process		cause					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Resveratrol: This phytochemical blocks the actions of a number of a number of cancer promoting genes thereby causing cancer cells to enter into apoptosis (cell death) and is included in the treatment of all cancers.	topic_ll
77579	4	356068	7	NULL	NULL	0	NULL	Resveratrol	Chemical		is used in the					cancer	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	Resveratrol: This phytochemical blocks the actions of a number of a number of cancer promoting genes thereby causing cancer cells to enter into apoptosis (cell death) and is included in the treatment of all cancers.	topic_ll
77580	5	356068	7	NULL	NULL	0	NULL	Resveratrol	Chemical		is a type of					phytochemical	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Resveratrol: This phytochemical blocks the actions of a number of a number of cancer promoting genes thereby causing cancer cells to enter into apoptosis (cell death) and is included in the treatment of all cancers.	topic_ll
77581	1	356069	7	NULL	NULL	0	NULL	MP	Chemical		role in		significant			AML	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the present study, together with our previous clinical experience, suggest that MP, especially at high doses, could have a significant role in the treatment of some AML patients by inducing apoptosis and differentiation of leukemic cells.	topic_ll
77582	2	356069	7	NULL	NULL	0	NULL	statement 1	Process		occur by					apoptosis	Process	inducing			NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the present study, together with our previous clinical experience, suggest that MP, especially at high doses, could have a significant role in the treatment of some AML patients by inducing apoptosis and differentiation of leukemic cells.	topic_ll
77583	3	356069	7	NULL	NULL	0	NULL	statement 1	Process		occur by					leukemic cells	Cell	differentiation of			NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the present study, together with our previous clinical experience, suggest that MP, especially at high doses, could have a significant role in the treatment of some AML patients by inducing apoptosis and differentiation of leukemic cells.	topic_ll
77584	1	356070	7	NULL	NULL	0	NULL	Resveratrol	Chemical		is a type of					natural phytochemical	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Resveratrol (trans-3,5,4′-trihydroxystilbene) is a natural phytochemical found in grapes and wine. Numerous biological effects of resveratrol have been reported in the last 10 years. In this paper, the competitive inhibition of intracellular uptake of glucose and dehydroascorbic acid in U937 and HL-60 cells by resveratrol is reported.	topic_ll
77585	2	356070	7	NULL	NULL	0	NULL	statement 1	Process		found in					grapes	Food				NULL		0	NULL	NULL	NULL	NULL	NULL	Resveratrol (trans-3,5,4′-trihydroxystilbene) is a natural phytochemical found in grapes and wine. Numerous biological effects of resveratrol have been reported in the last 10 years. In this paper, the competitive inhibition of intracellular uptake of glucose and dehydroascorbic acid in U937 and HL-60 cells by resveratrol is reported.	topic_ll
77586	3	356070	7	NULL	NULL	0	NULL	statement 1	Process		found in					wine	Food				NULL		0	NULL	NULL	NULL	NULL	NULL	Resveratrol (trans-3,5,4′-trihydroxystilbene) is a natural phytochemical found in grapes and wine. Numerous biological effects of resveratrol have been reported in the last 10 years. In this paper, the competitive inhibition of intracellular uptake of glucose and dehydroascorbic acid in U937 and HL-60 cells by resveratrol is reported.	topic_ll
77587	4	356070	7	NULL	NULL	NULL	NULL	resveratrol 	Chemical		inhibits		competitively			glucose	Chemical	intracellular uptake of			NULL	U937 cells	NULL	NULL	NULL	NULL	NULL	NULL	Resveratrol (trans-3,5,4′-trihydroxystilbene) is a natural phytochemical found in grapes and wine. Numerous biological effects of resveratrol have been reported in the last 10 years. In this paper, the competitive inhibition of intracellular uptake of glucose and dehydroascorbic acid in U937 and HL-60 cells by resveratrol is reported.	topic_ll
77588	5	356070	7	NULL	NULL	NULL	NULL	resveratrol	Chemical		inhibits		competitively			dehydroascorbic acid	Chemical	intracellular uptake of			NULL	U937 cells	NULL	NULL	NULL	NULL	NULL	NULL	Resveratrol (trans-3,5,4′-trihydroxystilbene) is a natural phytochemical found in grapes and wine. Numerous biological effects of resveratrol have been reported in the last 10 years. In this paper, the competitive inhibition of intracellular uptake of glucose and dehydroascorbic acid in U937 and HL-60 cells by resveratrol is reported.	topic_ll
77589	6	356070	7	NULL	NULL	0	NULL	resveratrol	Chemical		inhibits		competitively			glucose	Chemical	intracellular uptake of			NULL	HL-60 cells	0	NULL	NULL	NULL	NULL	NULL	Resveratrol (trans-3,5,4′-trihydroxystilbene) is a natural phytochemical found in grapes and wine. Numerous biological effects of resveratrol have been reported in the last 10 years. In this paper, the competitive inhibition of intracellular uptake of glucose and dehydroascorbic acid in U937 and HL-60 cells by resveratrol is reported.	topic_ll
77590	7	356070	7	NULL	NULL	NULL	NULL	resveratrol	Chemical		inhibits		competitively			dehydroascorbic acid	Chemical	intracellular uptake of			NULL	HL-60 cells	NULL	NULL	NULL	NULL	NULL	NULL	Resveratrol (trans-3,5,4′-trihydroxystilbene) is a natural phytochemical found in grapes and wine. Numerous biological effects of resveratrol have been reported in the last 10 years. In this paper, the competitive inhibition of intracellular uptake of glucose and dehydroascorbic acid in U937 and HL-60 cells by resveratrol is reported.	topic_ll
77591	8	356070	7	NULL	NULL	0	NULL	resveratrol	Chemical		is					trans-3,5,4?-trihydroxystilbene	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Resveratrol (trans-3,5,4′-trihydroxystilbene) is a natural phytochemical found in grapes and wine. Numerous biological effects of resveratrol have been reported in the last 10 years. In this paper, the competitive inhibition of intracellular uptake of glucose and dehydroascorbic acid in U937 and HL-60 cells by resveratrol is reported.	topic_ll
77592	1	356071	7	NULL	NULL	NULL	NULL	mitochondrial respiration	Process	decreased	point to					mitochondria	CellComponent	underlying dysfunction of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Several pieces of evidence point to an underlying dysfunction of mitochondria: (i) decreased mitochondrial respiration; (ii) changes in mitochondrial morphology; (iii) increases in mitochondrial DNA (mtDNA) polymorphisms and in levels of mtDNA mutations; (iv) downregulation of nuclear mRNA molecules and proteins involved in mitochondrial respiration; (v) decreased high-energy phosphates and decreased pH in the brain; and (vi) psychotic and affective symptoms, and cognitive decline in mitochondrial disorders. 	topic_bd
77593	2	356071	7	NULL	NULL	0	NULL	mitochondrial morphology	PhysicalPhenomenon	changes in	point to					mitochondria	CellComponent	underlying dysfunction of			NULL		0	NULL	NULL	NULL	NULL	NULL	Several pieces of evidence point to an underlying dysfunction of mitochondria: (i) decreased mitochondrial respiration; (ii) changes in mitochondrial morphology; (iii) increases in mitochondrial DNA (mtDNA) polymorphisms and in levels of mtDNA mutations; (iv) downregulation of nuclear mRNA molecules and proteins involved in mitochondrial respiration; (v) decreased high-energy phosphates and decreased pH in the brain; and (vi) psychotic and affective symptoms, and cognitive decline in mitochondrial disorders. 	topic_bd
77594	3	356071	7	NULL	NULL	0	NULL	mtDNA	NucleicAcid	increase in	point to					mitochondria	CellComponent	underlying dysfunction of			NULL		0	NULL	NULL	NULL	NULL	NULL	Several pieces of evidence point to an underlying dysfunction of mitochondria: (i) decreased mitochondrial respiration; (ii) changes in mitochondrial morphology; (iii) increases in mitochondrial DNA (mtDNA) polymorphisms and in levels of mtDNA mutations; (iv) downregulation of nuclear mRNA molecules and proteins involved in mitochondrial respiration; (v) decreased high-energy phosphates and decreased pH in the brain; and (vi) psychotic and affective symptoms, and cognitive decline in mitochondrial disorders. 	topic_bd
77595	4	356071	7	NULL	NULL	0	NULL	mtDNA	NucleicAcid	increase in levels of mutation of	point to					mitochondria	CellComponent	underlying dysfunction of			NULL		0	NULL	NULL	NULL	NULL	NULL	Several pieces of evidence point to an underlying dysfunction of mitochondria: (i) decreased mitochondrial respiration; (ii) changes in mitochondrial morphology; (iii) increases in mitochondrial DNA (mtDNA) polymorphisms and in levels of mtDNA mutations; (iv) downregulation of nuclear mRNA molecules and proteins involved in mitochondrial respiration; (v) decreased high-energy phosphates and decreased pH in the brain; and (vi) psychotic and affective symptoms, and cognitive decline in mitochondrial disorders. 	topic_bd
77596	5	356071	7	NULL	NULL	NULL	NULL	 nuclear mRNA molecule	GP		involved in					mitochondrial respiration	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Several pieces of evidence point to an underlying dysfunction of mitochondria: (i) decreased mitochondrial respiration; (ii) changes in mitochondrial morphology; (iii) increases in mitochondrial DNA (mtDNA) polymorphisms and in levels of mtDNA mutations; (iv) downregulation of nuclear mRNA molecules and proteins involved in mitochondrial respiration; (v) decreased high-energy phosphates and decreased pH in the brain; and (vi) psychotic and affective symptoms, and cognitive decline in mitochondrial disorders. 	topic_bd
77597	6	356071	7	NULL	NULL	NULL	NULL	nuclear proteins	GP		involved in					mitochondrial respiration	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Several pieces of evidence point to an underlying dysfunction of mitochondria: (i) decreased mitochondrial respiration; (ii) changes in mitochondrial morphology; (iii) increases in mitochondrial DNA (mtDNA) polymorphisms and in levels of mtDNA mutations; (iv) downregulation of nuclear mRNA molecules and proteins involved in mitochondrial respiration; (v) decreased high-energy phosphates and decreased pH in the brain; and (vi) psychotic and affective symptoms, and cognitive decline in mitochondrial disorders. 	topic_bd
77598	7	356071	7	NULL	NULL	0	NULL	nuclear mRNA molecule	GP	downregulation of	point to					mitochondria	CellComponent	underlying dysfunction of			NULL		0	NULL	NULL	NULL	NULL	NULL	Several pieces of evidence point to an underlying dysfunction of mitochondria: (i) decreased mitochondrial respiration; (ii) changes in mitochondrial morphology; (iii) increases in mitochondrial DNA (mtDNA) polymorphisms and in levels of mtDNA mutations; (iv) downregulation of nuclear mRNA molecules and proteins involved in mitochondrial respiration; (v) decreased high-energy phosphates and decreased pH in the brain; and (vi) psychotic and affective symptoms, and cognitive decline in mitochondrial disorders. 	topic_bd
77599	8	356071	7	NULL	NULL	0	NULL	nuclear proteins	GP	downregulation of	point to					mitochondria	CellComponent	underlying dysfunction of			NULL		0	NULL	NULL	NULL	NULL	NULL	Several pieces of evidence point to an underlying dysfunction of mitochondria: (i) decreased mitochondrial respiration; (ii) changes in mitochondrial morphology; (iii) increases in mitochondrial DNA (mtDNA) polymorphisms and in levels of mtDNA mutations; (iv) downregulation of nuclear mRNA molecules and proteins involved in mitochondrial respiration; (v) decreased high-energy phosphates and decreased pH in the brain; and (vi) psychotic and affective symptoms, and cognitive decline in mitochondrial disorders. 	topic_bd
77600	9	356071	7	NULL	NULL	NULL	NULL	high energy phosphates	Chemical	decreased	point to					mitochondria	CellComponent	underlying dysfunction of			NULL	brain	NULL	NULL	NULL	NULL	NULL	NULL	Several pieces of evidence point to an underlying dysfunction of mitochondria: (i) decreased mitochondrial respiration; (ii) changes in mitochondrial morphology; (iii) increases in mitochondrial DNA (mtDNA) polymorphisms and in levels of mtDNA mutations; (iv) downregulation of nuclear mRNA molecules and proteins involved in mitochondrial respiration; (v) decreased high-energy phosphates and decreased pH in the brain; and (vi) psychotic and affective symptoms, and cognitive decline in mitochondrial disorders. 	topic_bd
77601	10	356071	7	NULL	NULL	NULL	NULL	pH	QuantityOrMeasure	decreased	point to					mitochondria	CellComponent	underlying dysfunction of			NULL	brain	NULL	NULL	NULL	NULL	NULL	NULL	Several pieces of evidence point to an underlying dysfunction of mitochondria: (i) decreased mitochondrial respiration; (ii) changes in mitochondrial morphology; (iii) increases in mitochondrial DNA (mtDNA) polymorphisms and in levels of mtDNA mutations; (iv) downregulation of nuclear mRNA molecules and proteins involved in mitochondrial respiration; (v) decreased high-energy phosphates and decreased pH in the brain; and (vi) psychotic and affective symptoms, and cognitive decline in mitochondrial disorders. 	topic_bd
77602	11	356071	7	NULL	NULL	0	NULL	mitochondrial disorder	MedicalFinding	psychotic symptoms in	point to					mitochondria	CellComponent	underlying dysfunction of			NULL		0	NULL	NULL	NULL	NULL	NULL	Several pieces of evidence point to an underlying dysfunction of mitochondria: (i) decreased mitochondrial respiration; (ii) changes in mitochondrial morphology; (iii) increases in mitochondrial DNA (mtDNA) polymorphisms and in levels of mtDNA mutations; (iv) downregulation of nuclear mRNA molecules and proteins involved in mitochondrial respiration; (v) decreased high-energy phosphates and decreased pH in the brain; and (vi) psychotic and affective symptoms, and cognitive decline in mitochondrial disorders. 	topic_bd
77603	12	356071	7	NULL	NULL	0	NULL	mitochondrial disorder	MedicalFinding	affective symptoms in	point to					mitochondria	CellComponent	underlying dysfunction of			NULL		0	NULL	NULL	NULL	NULL	NULL	Several pieces of evidence point to an underlying dysfunction of mitochondria: (i) decreased mitochondrial respiration; (ii) changes in mitochondrial morphology; (iii) increases in mitochondrial DNA (mtDNA) polymorphisms and in levels of mtDNA mutations; (iv) downregulation of nuclear mRNA molecules and proteins involved in mitochondrial respiration; (v) decreased high-energy phosphates and decreased pH in the brain; and (vi) psychotic and affective symptoms, and cognitive decline in mitochondrial disorders. 	topic_bd
77604	13	356071	7	NULL	NULL	0	NULL	mitochondrial disorder	MedicalFinding	cognitive decline in	point to					mitochondria	CellComponent	underlying dysfunction of			NULL		0	NULL	NULL	NULL	NULL	NULL	Several pieces of evidence point to an underlying dysfunction of mitochondria: (i) decreased mitochondrial respiration; (ii) changes in mitochondrial morphology; (iii) increases in mitochondrial DNA (mtDNA) polymorphisms and in levels of mtDNA mutations; (iv) downregulation of nuclear mRNA molecules and proteins involved in mitochondrial respiration; (v) decreased high-energy phosphates and decreased pH in the brain; and (vi) psychotic and affective symptoms, and cognitive decline in mitochondrial disorders. 	topic_bd
78062	1	356072	6	NULL	NULL	0	NULL	age	AbstractConcept		increases					Breast cancer	MedicalFinding	development of			NULL		0	NULL	NULL	NULL	NULL	NULL	Your risk of developing breast cancer increases as you get older. About 1 out of 8 invasive breast cancers are found in women younger than 45, while about 2 out of 3 invasive breast cancers are found in women age 55 or older.	topic_bc
78063	1	356072	6	NULL	NULL	0	NULL	age	AbstractConcept		increases					Breast cancer	MedicalFinding	development of			NULL		0	NULL	NULL	NULL	NULL	NULL	Your risk of developing breast cancer increases as you get older. About 1 out of 8 invasive breast cancers are found in women younger than 45, while about 2 out of 3 invasive breast cancers are found in women age 55 or older.	topic_bc
77605	1	356073	7	NULL	NULL	0	NULL	BPD susceptibility region	Chromosome		located at					3q29	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	We identified a bipolar disorder (BPD) susceptibility region on chromosome 3q29 in a genome-wide linkage scan ( Bailer et al. 2002 (Biol Psychiatry 52: 40), NPL-score 4.09) and follow-up linkage analysis ( Schosser et al. 2004 (J Psychiatr Res 38(3): 357), NPL-scores >3 with five markers). 	topic_bd
77606	2	356073	7	NULL	NULL	0	NULL	BPD	MedicalFinding		is					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We identified a bipolar disorder (BPD) susceptibility region on chromosome 3q29 in a genome-wide linkage scan ( Bailer et al. 2002 (Biol Psychiatry 52: 40), NPL-score 4.09) and follow-up linkage analysis ( Schosser et al. 2004 (J Psychiatr Res 38(3): 357), NPL-scores >3 with five markers). 	topic_bd
77607	1	356074	7	NULL	NULL	0	NULL	BPD susceptibility region	Chromosome		located at					3q29 	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	We identified a bipolar disorder (BPD) susceptibility region on chromosome 3q29 in a genome-wide linkage scan ( Bailer et al. 2002 (Biol Psychiatry 52: 40), NPL-score 4.09) and follow-up linkage analysis ( Schosser et al. 2004 (J Psychiatr Res 38(3): 357), NPL-scores >3 with five markers). These findings were supported by further fine-mapping of this region ( Schosser et al. 2007 (Eur Neuropsychopharmacol 17(6-7): 501)), finding NPL-scores >3.9 with SNPs (single nucleotide polymorphisms) spanning a region of 3.46 Mbp in BPD families. Since genetic association studies are more powerful than linkage studies for detecting susceptibility genes of small effect size, we aimed to replicate these findings in an independent case-control sample collected in London (UK) and Vienna (Austria). Methods. A total of 51 SNPs were genotyped using Sequenom MassARRAY(®) iPLEX Gold and tested for association in a sample of 526 cases suffering from DSM-IV and/or ICD-10 diagnosis of BPD and 691 controls. Results. No genotypic and/or allelic association, as well as no haplotypic association, was found for any SNP after multiple testing correction. Conclusions. However, we cannot exclude the possibility that our sample might not have the power to detect rare variants associated with susceptibility to BPD.	topic_bd
77608	2	356074	7	NULL	NULL	0	NULL	BPD	MedicalFinding		is					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We identified a bipolar disorder (BPD) susceptibility region on chromosome 3q29 in a genome-wide linkage scan ( Bailer et al. 2002 (Biol Psychiatry 52: 40), NPL-score 4.09) and follow-up linkage analysis ( Schosser et al. 2004 (J Psychiatr Res 38(3): 357), NPL-scores >3 with five markers). These findings were supported by further fine-mapping of this region ( Schosser et al. 2007 (Eur Neuropsychopharmacol 17(6-7): 501)), finding NPL-scores >3.9 with SNPs (single nucleotide polymorphisms) spanning a region of 3.46 Mbp in BPD families. Since genetic association studies are more powerful than linkage studies for detecting susceptibility genes of small effect size, we aimed to replicate these findings in an independent case-control sample collected in London (UK) and Vienna (Austria). Methods. A total of 51 SNPs were genotyped using Sequenom MassARRAY(®) iPLEX Gold and tested for association in a sample of 526 cases suffering from DSM-IV and/or ICD-10 diagnosis of BPD and 691 controls. Results. No genotypic and/or allelic association, as well as no haplotypic association, was found for any SNP after multiple testing correction. Conclusions. However, we cannot exclude the possibility that our sample might not have the power to detect rare variants associated with susceptibility to BPD.	topic_bd
77609	1	356075	7	NULL	NULL	0	NULL	 transcriptome	NucleicAcid		is the set of					RNA molecules	NucleicAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	The transcriptome is the set of all RNA molecules, including mRNA, rRNA, tRNA, and other non-coding RNA produced in one or a population of cells.	topic_bd
77610	2	356075	7	NULL	NULL	0	NULL	RNA molecules	NucleicAcid		include					mRNA	NucleicAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	The transcriptome is the set of all RNA molecules, including mRNA, rRNA, tRNA, and other non-coding RNA produced in one or a population of cells.	topic_bd
77611	3	356075	7	NULL	NULL	0	NULL	RNA molecules	NucleicAcid		include					rRNA	NucleicAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	The transcriptome is the set of all RNA molecules, including mRNA, rRNA, tRNA, and other non-coding RNA produced in one or a population of cells.	topic_bd
77612	4	356075	7	NULL	NULL	0	NULL	RNA molecules	NucleicAcid		include					tRNA	NucleicAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	The transcriptome is the set of all RNA molecules, including mRNA, rRNA, tRNA, and other non-coding RNA produced in one or a population of cells.	topic_bd
77613	5	356075	7	NULL	NULL	0	NULL	RNA molecules	NucleicAcid		include					non-coding RNA	NucleicAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	The transcriptome is the set of all RNA molecules, including mRNA, rRNA, tRNA, and other non-coding RNA produced in one or a population of cells.	topic_bd
77614	6	356075	7	NULL	NULL	NULL	NULL	statement 1	NucleicAcid		occur in					cells	Cell	population of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	The transcriptome is the set of all RNA molecules, including mRNA, rRNA, tRNA, and other non-coding RNA produced in one or a population of cells.	topic_bd
77615	7	356075	7	NULL	NULL	NULL	NULL	statement 1	NucleicAcid		occur in					one cell	Cell				NULL		NULL	NULL	NULL	NULL	NULL	NULL	The transcriptome is the set of all RNA molecules, including mRNA, rRNA, tRNA, and other non-coding RNA produced in one or a population of cells.	topic_bd
77616	8	356075	7	NULL	NULL	0	NULL	statement 6	Process		is an alternative to					statement 7	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The transcriptome is the set of all RNA molecules, including mRNA, rRNA, tRNA, and other non-coding RNA produced in one or a population of cells.	topic_bd
77617	1	356076	7	NULL	NULL	0	NULL	Transcriptome	NucleicAcid		refers to					mRNAs	NucleicAcid	entirety of			NULL		0	NULL	NULL	NULL	NULL	NULL	‘Transcriptome’ refers to the entirety of messenger ribonucleic acids (mRNAs) in a particular tissue. It is assumed that an altered expression level of an mRNA in a disease is an indication for an abnormality in either the encoded protein, or a biologically connected structure or function. I	topic_bd
77618	2	356076	7	NULL	NULL	0	NULL	statement 1	NucleicAcid		occur in					tissue	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	‘Transcriptome’ refers to the entirety of messenger ribonucleic acids (mRNAs) in a particular tissue. It is assumed that an altered expression level of an mRNA in a disease is an indication for an abnormality in either the encoded protein, or a biologically connected structure or function. I	topic_bd
77619	3	356076	7	NULL	NULL	NULL	NULL	mRNA	NucleicAcid	altered expression level of 	indicate					encoded protein	GP	abnormality in			NULL		NULL	NULL	NULL	NULL	NULL	NULL	‘Transcriptome’ refers to the entirety of messenger ribonucleic acids (mRNAs) in a particular tissue. It is assumed that an altered expression level of an mRNA in a disease is an indication for an abnormality in either the encoded protein, or a biologically connected structure or function. I	topic_bd
77620	4	356076	7	NULL	NULL	0	NULL	statement 3	Process		occur in a					disease	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	‘Transcriptome’ refers to the entirety of messenger ribonucleic acids (mRNAs) in a particular tissue. It is assumed that an altered expression level of an mRNA in a disease is an indication for an abnormality in either the encoded protein, or a biologically connected structure or function. I	topic_bd
77621	5	356076	7	NULL	NULL	0	NULL	mRNA	NucleicAcid	altered expression level of 	indicate					biologically connected structure	CellComponent	abnormality in			NULL		0	NULL	NULL	NULL	NULL	NULL	‘Transcriptome’ refers to the entirety of messenger ribonucleic acids (mRNAs) in a particular tissue. It is assumed that an altered expression level of an mRNA in a disease is an indication for an abnormality in either the encoded protein, or a biologically connected structure or function. I	topic_bd
77622	6	356076	7	NULL	NULL	0	NULL	mRNA	NucleicAcid	altered expression level of 	indicate					biological function	Process	abnormality in			NULL		0	NULL	NULL	NULL	NULL	NULL	‘Transcriptome’ refers to the entirety of messenger ribonucleic acids (mRNAs) in a particular tissue. It is assumed that an altered expression level of an mRNA in a disease is an indication for an abnormality in either the encoded protein, or a biologically connected structure or function. I	topic_bd
77623	7	356076	7	NULL	NULL	0	NULL	statement 5	Process		occur in a					disease	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	‘Transcriptome’ refers to the entirety of messenger ribonucleic acids (mRNAs) in a particular tissue. It is assumed that an altered expression level of an mRNA in a disease is an indication for an abnormality in either the encoded protein, or a biologically connected structure or function. I	topic_bd
77624	8	356076	7	NULL	NULL	0	NULL	statement 6	Process		occur in a					disease	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	‘Transcriptome’ refers to the entirety of messenger ribonucleic acids (mRNAs) in a particular tissue. It is assumed that an altered expression level of an mRNA in a disease is an indication for an abnormality in either the encoded protein, or a biologically connected structure or function. I	topic_bd
77625	9	356076	7	NULL	NULL	0	NULL	mRNA	NucleicAcid		is					messenger ribonucleic acids	NucleicAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	‘Transcriptome’ refers to the entirety of messenger ribonucleic acids (mRNAs) in a particular tissue. It is assumed that an altered expression level of an mRNA in a disease is an indication for an abnormality in either the encoded protein, or a biologically connected structure or function. I	topic_bd
78176	1	356077	6	NULL	NULL	0	NULL	miR-126	NucleicAcid	restoration of	reduces					tumour growth	process				NULL		0	NULL	NULL	NULL	NULL	NULL	A search for general regulators of cancer metastasis has yielded a set of microRNAs for which expression is specifically lost as human breast cancer cells develop metastatic potential. Here we show that restoring the expression of these microRNAs in malignant cells suppresses lung and bone metastasis by human cancer cells in vivo. Of these microRNAs, miR-126 restoration reduces overall tumour growth and proliferation, whereas miR-335 inhibits metastatic cell invasion. miR-335 regulates a set of genes whose collective expression in a large cohort of human tumours is associated with risk of distal metastasis. miR-335 suppresses metastasis and migration through targeting of the progenitor cell transcription factor SOX4 and extracellular matrix component tenascin C. Expression of miR-126 and miR-335 is lost in the majority of primary breast tumours from patients who relapse, and the loss of expression of either microRNA is associated with poor distal metastasis-free survival. miR-335 and miR-126 are thus identified as metastasis suppressor microRNAs in human breast cancer.	topic_bc
78177	2	356077	6	NULL	NULL	0	NULL	miR-126	NucleicAcid		reduces					tumour proliferation	process				NULL		0	NULL	NULL	NULL	NULL	NULL	A search for general regulators of cancer metastasis has yielded a set of microRNAs for which expression is specifically lost as human breast cancer cells develop metastatic potential. Here we show that restoring the expression of these microRNAs in malignant cells suppresses lung and bone metastasis by human cancer cells in vivo. Of these microRNAs, miR-126 restoration reduces overall tumour growth and proliferation, whereas miR-335 inhibits metastatic cell invasion. miR-335 regulates a set of genes whose collective expression in a large cohort of human tumours is associated with risk of distal metastasis. miR-335 suppresses metastasis and migration through targeting of the progenitor cell transcription factor SOX4 and extracellular matrix component tenascin C. Expression of miR-126 and miR-335 is lost in the majority of primary breast tumours from patients who relapse, and the loss of expression of either microRNA is associated with poor distal metastasis-free survival. miR-335 and miR-126 are thus identified as metastasis suppressor microRNAs in human breast cancer.	topic_bc
78178	3	356077	6	NULL	NULL	0	NULL	miR-335	NucleicAcid		inhibits					metastatic cell	cell	invasion of 			NULL		0	NULL	NULL	NULL	NULL	NULL	A search for general regulators of cancer metastasis has yielded a set of microRNAs for which expression is specifically lost as human breast cancer cells develop metastatic potential. Here we show that restoring the expression of these microRNAs in malignant cells suppresses lung and bone metastasis by human cancer cells in vivo. Of these microRNAs, miR-126 restoration reduces overall tumour growth and proliferation, whereas miR-335 inhibits metastatic cell invasion. miR-335 regulates a set of genes whose collective expression in a large cohort of human tumours is associated with risk of distal metastasis. miR-335 suppresses metastasis and migration through targeting of the progenitor cell transcription factor SOX4 and extracellular matrix component tenascin C. Expression of miR-126 and miR-335 is lost in the majority of primary breast tumours from patients who relapse, and the loss of expression of either microRNA is associated with poor distal metastasis-free survival. miR-335 and miR-126 are thus identified as metastasis suppressor microRNAs in human breast cancer.	topic_bc
78179	4	356077	6	NULL	NULL	0	NULL	SOX4	GP		is a type of					progenitor cell transcription factor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	A search for general regulators of cancer metastasis has yielded a set of microRNAs for which expression is specifically lost as human breast cancer cells develop metastatic potential. Here we show that restoring the expression of these microRNAs in malignant cells suppresses lung and bone metastasis by human cancer cells in vivo. Of these microRNAs, miR-126 restoration reduces overall tumour growth and proliferation, whereas miR-335 inhibits metastatic cell invasion. miR-335 regulates a set of genes whose collective expression in a large cohort of human tumours is associated with risk of distal metastasis. miR-335 suppresses metastasis and migration through targeting of the progenitor cell transcription factor SOX4 and extracellular matrix component tenascin C. Expression of miR-126 and miR-335 is lost in the majority of primary breast tumours from patients who relapse, and the loss of expression of either microRNA is associated with poor distal metastasis-free survival. miR-335 and miR-126 are thus identified as metastasis suppressor microRNAs in human breast cancer.	topic_bc
78180	5	356077	6	NULL	NULL	0	NULL	 tenascin C	GP		is a type of					 extracellular matrix component	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	A search for general regulators of cancer metastasis has yielded a set of microRNAs for which expression is specifically lost as human breast cancer cells develop metastatic potential. Here we show that restoring the expression of these microRNAs in malignant cells suppresses lung and bone metastasis by human cancer cells in vivo. Of these microRNAs, miR-126 restoration reduces overall tumour growth and proliferation, whereas miR-335 inhibits metastatic cell invasion. miR-335 regulates a set of genes whose collective expression in a large cohort of human tumours is associated with risk of distal metastasis. miR-335 suppresses metastasis and migration through targeting of the progenitor cell transcription factor SOX4 and extracellular matrix component tenascin C. Expression of miR-126 and miR-335 is lost in the majority of primary breast tumours from patients who relapse, and the loss of expression of either microRNA is associated with poor distal metastasis-free survival. miR-335 and miR-126 are thus identified as metastasis suppressor microRNAs in human breast cancer.	topic_bc
78171	1	356080	6	NULL	NULL	0	NULL	rs4415084	NucleicAcid		is located on					chromosome 5p12	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	We carried out a genome-wide association study of breast cancer predisposition with replication and refinement studies involving 6,145 cases and 33,016 controls and identified two SNPs (rs4415084 and rs10941679) on 5p12 that confer risk, preferentially for estrogen receptor (ER)-positive tumors (OR = 1.27, P = 2.5 × 10−12 for rs10941679). The nearest gene, MRPS30, was previously implicated in apoptosis, ER-positive tumors and favorable prognosis. A recently reported signal in FGFR2 was also found to associate specifically with ER-positive breast cancer. http://www.nature.com/ng/journal/v40/n6/full/ng.131.html	topic_bc
78172	2	356080	6	NULL	NULL	0	NULL	rs10941679	NucleicAcid		is located on					chromosome 5p12	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	We carried out a genome-wide association study of breast cancer predisposition with replication and refinement studies involving 6,145 cases and 33,016 controls and identified two SNPs (rs4415084 and rs10941679) on 5p12 that confer risk, preferentially for estrogen receptor (ER)-positive tumors (OR = 1.27, P = 2.5 × 10−12 for rs10941679). The nearest gene, MRPS30, was previously implicated in apoptosis, ER-positive tumors and favorable prognosis. A recently reported signal in FGFR2 was also found to associate specifically with ER-positive breast cancer. http://www.nature.com/ng/journal/v40/n6/full/ng.131.html	topic_bc
78173	3	356080	6	NULL	NULL	0	NULL	statement 1	process		poses risk for					ER positive tumors	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We carried out a genome-wide association study of breast cancer predisposition with replication and refinement studies involving 6,145 cases and 33,016 controls and identified two SNPs (rs4415084 and rs10941679) on 5p12 that confer risk, preferentially for estrogen receptor (ER)-positive tumors (OR = 1.27, P = 2.5 × 10−12 for rs10941679). The nearest gene, MRPS30, was previously implicated in apoptosis, ER-positive tumors and favorable prognosis. A recently reported signal in FGFR2 was also found to associate specifically with ER-positive breast cancer. http://www.nature.com/ng/journal/v40/n6/full/ng.131.html	topic_bc
78174	4	356080	6	NULL	NULL	0	NULL	statement 2	process		poses risk for					ER positive tumors	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We carried out a genome-wide association study of breast cancer predisposition with replication and refinement studies involving 6,145 cases and 33,016 controls and identified two SNPs (rs4415084 and rs10941679) on 5p12 that confer risk, preferentially for estrogen receptor (ER)-positive tumors (OR = 1.27, P = 2.5 × 10−12 for rs10941679). The nearest gene, MRPS30, was previously implicated in apoptosis, ER-positive tumors and favorable prognosis. A recently reported signal in FGFR2 was also found to associate specifically with ER-positive breast cancer. http://www.nature.com/ng/journal/v40/n6/full/ng.131.html	topic_bc
78175	5	356080	6	NULL	NULL	0	NULL	MRPS30	GP		is implicated in					apoptosis	process				NULL		0	NULL	NULL	NULL	NULL	NULL	We carried out a genome-wide association study of breast cancer predisposition with replication and refinement studies involving 6,145 cases and 33,016 controls and identified two SNPs (rs4415084 and rs10941679) on 5p12 that confer risk, preferentially for estrogen receptor (ER)-positive tumors (OR = 1.27, P = 2.5 × 10−12 for rs10941679). The nearest gene, MRPS30, was previously implicated in apoptosis, ER-positive tumors and favorable prognosis. A recently reported signal in FGFR2 was also found to associate specifically with ER-positive breast cancer. http://www.nature.com/ng/journal/v40/n6/full/ng.131.html	topic_bc
78167	1	356081	6	NULL	NULL	0	NULL	Mesenchymal stem cells	Cell		localize					breast carcinoma	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Mesenchymal stem cells have been recently described to localize to breast carcinomas, where they integrate into the tumour-associated stroma. However, the involvement of mesenchymal stem cells (or their derivatives) in tumour pathophysiology has not been addressed. Here, we demonstrate that bone-marrow-derived human mesenchymal stem cells, when mixed with otherwise weakly metastatic human breast carcinoma cells, cause the cancer cells to increase their metastatic potency greatly when this cell mixture is introduced into a subcutaneous site and allowed to form a tumour xenograft. The breast cancer cells stimulate de novo secretion of the chemokine CCL5 (also called RANTES) from mesenchymal stem cells, which then acts in a paracrine fashion on the cancer cells to enhance their motility, invasion and metastasis. This enhanced metastatic ability is reversible and is dependent on CCL5 signalling through the chemokine receptor CCR5. Collectively, these data demonstrate that the tumour microenvironment facilitates metastatic spread by eliciting reversible changes in the phenotype of cancer cells.	topic_bc
78168	2	356081	6	NULL	NULL	0	NULL	breast cancer cell	Cell		stimulate					CCL5	Chemical	secretion of			NULL	de novo	0	NULL	NULL	NULL	NULL	NULL	Mesenchymal stem cells have been recently described to localize to breast carcinomas, where they integrate into the tumour-associated stroma. However, the involvement of mesenchymal stem cells (or their derivatives) in tumour pathophysiology has not been addressed. Here, we demonstrate that bone-marrow-derived human mesenchymal stem cells, when mixed with otherwise weakly metastatic human breast carcinoma cells, cause the cancer cells to increase their metastatic potency greatly when this cell mixture is introduced into a subcutaneous site and allowed to form a tumour xenograft. The breast cancer cells stimulate de novo secretion of the chemokine CCL5 (also called RANTES) from mesenchymal stem cells, which then acts in a paracrine fashion on the cancer cells to enhance their motility, invasion and metastasis. This enhanced metastatic ability is reversible and is dependent on CCL5 signalling through the chemokine receptor CCR5. Collectively, these data demonstrate that the tumour microenvironment facilitates metastatic spread by eliciting reversible changes in the phenotype of cancer cells.	topic_bc
78169	3	356081	6	NULL	NULL	0	NULL	CCL5	Chemical		is a type of					chemokine	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Mesenchymal stem cells have been recently described to localize to breast carcinomas, where they integrate into the tumour-associated stroma. However, the involvement of mesenchymal stem cells (or their derivatives) in tumour pathophysiology has not been addressed. Here, we demonstrate that bone-marrow-derived human mesenchymal stem cells, when mixed with otherwise weakly metastatic human breast carcinoma cells, cause the cancer cells to increase their metastatic potency greatly when this cell mixture is introduced into a subcutaneous site and allowed to form a tumour xenograft. The breast cancer cells stimulate de novo secretion of the chemokine CCL5 (also called RANTES) from mesenchymal stem cells, which then acts in a paracrine fashion on the cancer cells to enhance their motility, invasion and metastasis. This enhanced metastatic ability is reversible and is dependent on CCL5 signalling through the chemokine receptor CCR5. Collectively, these data demonstrate that the tumour microenvironment facilitates metastatic spread by eliciting reversible changes in the phenotype of cancer cells.	topic_bc
78170	4	356081	6	NULL	NULL	0	NULL	CCL5	Chemical		is					RANTES	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Mesenchymal stem cells have been recently described to localize to breast carcinomas, where they integrate into the tumour-associated stroma. However, the involvement of mesenchymal stem cells (or their derivatives) in tumour pathophysiology has not been addressed. Here, we demonstrate that bone-marrow-derived human mesenchymal stem cells, when mixed with otherwise weakly metastatic human breast carcinoma cells, cause the cancer cells to increase their metastatic potency greatly when this cell mixture is introduced into a subcutaneous site and allowed to form a tumour xenograft. The breast cancer cells stimulate de novo secretion of the chemokine CCL5 (also called RANTES) from mesenchymal stem cells, which then acts in a paracrine fashion on the cancer cells to enhance their motility, invasion and metastasis. This enhanced metastatic ability is reversible and is dependent on CCL5 signalling through the chemokine receptor CCR5. Collectively, these data demonstrate that the tumour microenvironment facilitates metastatic spread by eliciting reversible changes in the phenotype of cancer cells.	topic_bc
78122	1	356084	6	NULL	NULL	0	NULL	VEGF	GP		is					vascular endothelial growth factor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	nvironmental chemicals may affect human health by disrupting endocrine function. Their possible role in the mammary gland and breast tumors is still unknown. Previous studies have demonstrated that vascular endothelial growth factor (VEGF), a key factor in angiogenesis and tumor progression, is an estrogen-regulated gene. We analyzed whether VEGF expression is regulated by different xenoestrogens in several breast cancer cells, MELN (derived from MCF-7) and MELP (derived from MDA-MB-231) and stably expressing estrogen receptor  (ER); these cell lines stably express estrogen response element (β-globin)-luciferase. Genistein, bisphenol A (BPA), 4-(tert-octyl)phenol (OP), dieldrin, and several phthalates, including benzyl butyl phthalate (BBP) and di-ethyl-2-hexyle phthalate (DEHP), were first shown to be estrogenic. These compounds induced a dose-dependent increase of VEGF secretion in MELN and MCF-7 cells; maximal effect was observed at 1–10 µM non-cytotoxic concentrations and was inhibited by the antiestrogen ICI 182 780. VEGF increase was not observed in ER-negative MDA-MB-231 cells. Most substances increased VEGF transcript levels in MELN cells. In contrast, -hexachlorocyclohexane, vinclozolin, and the phthalates (mono-n-butyl ester phthalic acid, di-isononyle phthalate, and di-isodecyle phthalate) were ineffective on both VEGF secretion and estrogenic luciferase induction in these cell lines. Specific kinase inhibitors PD98059, SB203580, or LY294002 suppressed the xenoestrogen-induced VEGF response, suggesting activation of MEK, p38 kinase, and phosphatidylinositol-3-kinase pathways. Our in vitro results show for the first time that genistein and xenoestrogens (BPA, OP, dieldrin, BBP, and DEHP at high concentrations) up-regulate VEGF expression in MELN cells by an ER-dependent mechanism. Since VEGF increases capillary permeability and breast tumor angiogenesis in vivo, the physiological relevance of these findings is discussed. http://joe.endocrinology-journals.org/cgi/content/abstract/196/2/399	topic_bc
78123	2	356084	6	NULL	NULL	0	NULL	VEGF	GP		plays a role in					angiogenesis	process				NULL		0	NULL	NULL	NULL	NULL	NULL	nvironmental chemicals may affect human health by disrupting endocrine function. Their possible role in the mammary gland and breast tumors is still unknown. Previous studies have demonstrated that vascular endothelial growth factor (VEGF), a key factor in angiogenesis and tumor progression, is an estrogen-regulated gene. We analyzed whether VEGF expression is regulated by different xenoestrogens in several breast cancer cells, MELN (derived from MCF-7) and MELP (derived from MDA-MB-231) and stably expressing estrogen receptor  (ER); these cell lines stably express estrogen response element (β-globin)-luciferase. Genistein, bisphenol A (BPA), 4-(tert-octyl)phenol (OP), dieldrin, and several phthalates, including benzyl butyl phthalate (BBP) and di-ethyl-2-hexyle phthalate (DEHP), were first shown to be estrogenic. These compounds induced a dose-dependent increase of VEGF secretion in MELN and MCF-7 cells; maximal effect was observed at 1–10 µM non-cytotoxic concentrations and was inhibited by the antiestrogen ICI 182 780. VEGF increase was not observed in ER-negative MDA-MB-231 cells. Most substances increased VEGF transcript levels in MELN cells. In contrast, -hexachlorocyclohexane, vinclozolin, and the phthalates (mono-n-butyl ester phthalic acid, di-isononyle phthalate, and di-isodecyle phthalate) were ineffective on both VEGF secretion and estrogenic luciferase induction in these cell lines. Specific kinase inhibitors PD98059, SB203580, or LY294002 suppressed the xenoestrogen-induced VEGF response, suggesting activation of MEK, p38 kinase, and phosphatidylinositol-3-kinase pathways. Our in vitro results show for the first time that genistein and xenoestrogens (BPA, OP, dieldrin, BBP, and DEHP at high concentrations) up-regulate VEGF expression in MELN cells by an ER-dependent mechanism. Since VEGF increases capillary permeability and breast tumor angiogenesis in vivo, the physiological relevance of these findings is discussed. http://joe.endocrinology-journals.org/cgi/content/abstract/196/2/399	topic_bc
78124	3	356084	6	NULL	NULL	0	NULL	VEGF	GP		plays a role in					tumor	MedicalFinding	progression of			NULL		0	NULL	NULL	NULL	NULL	NULL	nvironmental chemicals may affect human health by disrupting endocrine function. Their possible role in the mammary gland and breast tumors is still unknown. Previous studies have demonstrated that vascular endothelial growth factor (VEGF), a key factor in angiogenesis and tumor progression, is an estrogen-regulated gene. We analyzed whether VEGF expression is regulated by different xenoestrogens in several breast cancer cells, MELN (derived from MCF-7) and MELP (derived from MDA-MB-231) and stably expressing estrogen receptor  (ER); these cell lines stably express estrogen response element (β-globin)-luciferase. Genistein, bisphenol A (BPA), 4-(tert-octyl)phenol (OP), dieldrin, and several phthalates, including benzyl butyl phthalate (BBP) and di-ethyl-2-hexyle phthalate (DEHP), were first shown to be estrogenic. These compounds induced a dose-dependent increase of VEGF secretion in MELN and MCF-7 cells; maximal effect was observed at 1–10 µM non-cytotoxic concentrations and was inhibited by the antiestrogen ICI 182 780. VEGF increase was not observed in ER-negative MDA-MB-231 cells. Most substances increased VEGF transcript levels in MELN cells. In contrast, -hexachlorocyclohexane, vinclozolin, and the phthalates (mono-n-butyl ester phthalic acid, di-isononyle phthalate, and di-isodecyle phthalate) were ineffective on both VEGF secretion and estrogenic luciferase induction in these cell lines. Specific kinase inhibitors PD98059, SB203580, or LY294002 suppressed the xenoestrogen-induced VEGF response, suggesting activation of MEK, p38 kinase, and phosphatidylinositol-3-kinase pathways. Our in vitro results show for the first time that genistein and xenoestrogens (BPA, OP, dieldrin, BBP, and DEHP at high concentrations) up-regulate VEGF expression in MELN cells by an ER-dependent mechanism. Since VEGF increases capillary permeability and breast tumor angiogenesis in vivo, the physiological relevance of these findings is discussed. http://joe.endocrinology-journals.org/cgi/content/abstract/196/2/399	topic_bc
78125	4	356084	6	NULL	NULL	0	NULL	VEGF	GP		is regulated by					estrogen	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	nvironmental chemicals may affect human health by disrupting endocrine function. Their possible role in the mammary gland and breast tumors is still unknown. Previous studies have demonstrated that vascular endothelial growth factor (VEGF), a key factor in angiogenesis and tumor progression, is an estrogen-regulated gene. We analyzed whether VEGF expression is regulated by different xenoestrogens in several breast cancer cells, MELN (derived from MCF-7) and MELP (derived from MDA-MB-231) and stably expressing estrogen receptor  (ER); these cell lines stably express estrogen response element (β-globin)-luciferase. Genistein, bisphenol A (BPA), 4-(tert-octyl)phenol (OP), dieldrin, and several phthalates, including benzyl butyl phthalate (BBP) and di-ethyl-2-hexyle phthalate (DEHP), were first shown to be estrogenic. These compounds induced a dose-dependent increase of VEGF secretion in MELN and MCF-7 cells; maximal effect was observed at 1–10 µM non-cytotoxic concentrations and was inhibited by the antiestrogen ICI 182 780. VEGF increase was not observed in ER-negative MDA-MB-231 cells. Most substances increased VEGF transcript levels in MELN cells. In contrast, -hexachlorocyclohexane, vinclozolin, and the phthalates (mono-n-butyl ester phthalic acid, di-isononyle phthalate, and di-isodecyle phthalate) were ineffective on both VEGF secretion and estrogenic luciferase induction in these cell lines. Specific kinase inhibitors PD98059, SB203580, or LY294002 suppressed the xenoestrogen-induced VEGF response, suggesting activation of MEK, p38 kinase, and phosphatidylinositol-3-kinase pathways. Our in vitro results show for the first time that genistein and xenoestrogens (BPA, OP, dieldrin, BBP, and DEHP at high concentrations) up-regulate VEGF expression in MELN cells by an ER-dependent mechanism. Since VEGF increases capillary permeability and breast tumor angiogenesis in vivo, the physiological relevance of these findings is discussed. http://joe.endocrinology-journals.org/cgi/content/abstract/196/2/399	topic_bc
78127	5	356084	6	NULL	NULL	0	NULL	Genistein	Chemical		increase					VEGF	GP	secretion of			NULL	MELN cells	0	NULL	NULL	NULL	NULL	NULL	nvironmental chemicals may affect human health by disrupting endocrine function. Their possible role in the mammary gland and breast tumors is still unknown. Previous studies have demonstrated that vascular endothelial growth factor (VEGF), a key factor in angiogenesis and tumor progression, is an estrogen-regulated gene. We analyzed whether VEGF expression is regulated by different xenoestrogens in several breast cancer cells, MELN (derived from MCF-7) and MELP (derived from MDA-MB-231) and stably expressing estrogen receptor  (ER); these cell lines stably express estrogen response element (β-globin)-luciferase. Genistein, bisphenol A (BPA), 4-(tert-octyl)phenol (OP), dieldrin, and several phthalates, including benzyl butyl phthalate (BBP) and di-ethyl-2-hexyle phthalate (DEHP), were first shown to be estrogenic. These compounds induced a dose-dependent increase of VEGF secretion in MELN and MCF-7 cells; maximal effect was observed at 1–10 µM non-cytotoxic concentrations and was inhibited by the antiestrogen ICI 182 780. VEGF increase was not observed in ER-negative MDA-MB-231 cells. Most substances increased VEGF transcript levels in MELN cells. In contrast, -hexachlorocyclohexane, vinclozolin, and the phthalates (mono-n-butyl ester phthalic acid, di-isononyle phthalate, and di-isodecyle phthalate) were ineffective on both VEGF secretion and estrogenic luciferase induction in these cell lines. Specific kinase inhibitors PD98059, SB203580, or LY294002 suppressed the xenoestrogen-induced VEGF response, suggesting activation of MEK, p38 kinase, and phosphatidylinositol-3-kinase pathways. Our in vitro results show for the first time that genistein and xenoestrogens (BPA, OP, dieldrin, BBP, and DEHP at high concentrations) up-regulate VEGF expression in MELN cells by an ER-dependent mechanism. Since VEGF increases capillary permeability and breast tumor angiogenesis in vivo, the physiological relevance of these findings is discussed. http://joe.endocrinology-journals.org/cgi/content/abstract/196/2/399	topic_bc
78129	6	356084	6	NULL	NULL	NULL	NULL	BPA	Chemical		increases					VEGF	GP	secretion of			NULL	MELN cells	NULL	NULL	NULL	NULL	NULL	NULL	nvironmental chemicals may affect human health by disrupting endocrine function. Their possible role in the mammary gland and breast tumors is still unknown. Previous studies have demonstrated that vascular endothelial growth factor (VEGF), a key factor in angiogenesis and tumor progression, is an estrogen-regulated gene. We analyzed whether VEGF expression is regulated by different xenoestrogens in several breast cancer cells, MELN (derived from MCF-7) and MELP (derived from MDA-MB-231) and stably expressing estrogen receptor  (ER); these cell lines stably express estrogen response element (β-globin)-luciferase. Genistein, bisphenol A (BPA), 4-(tert-octyl)phenol (OP), dieldrin, and several phthalates, including benzyl butyl phthalate (BBP) and di-ethyl-2-hexyle phthalate (DEHP), were first shown to be estrogenic. These compounds induced a dose-dependent increase of VEGF secretion in MELN and MCF-7 cells; maximal effect was observed at 1–10 µM non-cytotoxic concentrations and was inhibited by the antiestrogen ICI 182 780. VEGF increase was not observed in ER-negative MDA-MB-231 cells. Most substances increased VEGF transcript levels in MELN cells. In contrast, -hexachlorocyclohexane, vinclozolin, and the phthalates (mono-n-butyl ester phthalic acid, di-isononyle phthalate, and di-isodecyle phthalate) were ineffective on both VEGF secretion and estrogenic luciferase induction in these cell lines. Specific kinase inhibitors PD98059, SB203580, or LY294002 suppressed the xenoestrogen-induced VEGF response, suggesting activation of MEK, p38 kinase, and phosphatidylinositol-3-kinase pathways. Our in vitro results show for the first time that genistein and xenoestrogens (BPA, OP, dieldrin, BBP, and DEHP at high concentrations) up-regulate VEGF expression in MELN cells by an ER-dependent mechanism. Since VEGF increases capillary permeability and breast tumor angiogenesis in vivo, the physiological relevance of these findings is discussed. http://joe.endocrinology-journals.org/cgi/content/abstract/196/2/399	topic_bc
78130	7	356084	6	NULL	NULL	NULL	NULL	OP	Chemical		increases					VEGF	GP	secretion of			NULL	MELN cells	NULL	NULL	NULL	NULL	NULL	NULL	nvironmental chemicals may affect human health by disrupting endocrine function. Their possible role in the mammary gland and breast tumors is still unknown. Previous studies have demonstrated that vascular endothelial growth factor (VEGF), a key factor in angiogenesis and tumor progression, is an estrogen-regulated gene. We analyzed whether VEGF expression is regulated by different xenoestrogens in several breast cancer cells, MELN (derived from MCF-7) and MELP (derived from MDA-MB-231) and stably expressing estrogen receptor  (ER); these cell lines stably express estrogen response element (β-globin)-luciferase. Genistein, bisphenol A (BPA), 4-(tert-octyl)phenol (OP), dieldrin, and several phthalates, including benzyl butyl phthalate (BBP) and di-ethyl-2-hexyle phthalate (DEHP), were first shown to be estrogenic. These compounds induced a dose-dependent increase of VEGF secretion in MELN and MCF-7 cells; maximal effect was observed at 1–10 µM non-cytotoxic concentrations and was inhibited by the antiestrogen ICI 182 780. VEGF increase was not observed in ER-negative MDA-MB-231 cells. Most substances increased VEGF transcript levels in MELN cells. In contrast, -hexachlorocyclohexane, vinclozolin, and the phthalates (mono-n-butyl ester phthalic acid, di-isononyle phthalate, and di-isodecyle phthalate) were ineffective on both VEGF secretion and estrogenic luciferase induction in these cell lines. Specific kinase inhibitors PD98059, SB203580, or LY294002 suppressed the xenoestrogen-induced VEGF response, suggesting activation of MEK, p38 kinase, and phosphatidylinositol-3-kinase pathways. Our in vitro results show for the first time that genistein and xenoestrogens (BPA, OP, dieldrin, BBP, and DEHP at high concentrations) up-regulate VEGF expression in MELN cells by an ER-dependent mechanism. Since VEGF increases capillary permeability and breast tumor angiogenesis in vivo, the physiological relevance of these findings is discussed. http://joe.endocrinology-journals.org/cgi/content/abstract/196/2/399	topic_bc
78132	8	356084	6	NULL	NULL	0	NULL	OP	GP		is					 4-(tert-octyl)phenol	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	nvironmental chemicals may affect human health by disrupting endocrine function. Their possible role in the mammary gland and breast tumors is still unknown. Previous studies have demonstrated that vascular endothelial growth factor (VEGF), a key factor in angiogenesis and tumor progression, is an estrogen-regulated gene. We analyzed whether VEGF expression is regulated by different xenoestrogens in several breast cancer cells, MELN (derived from MCF-7) and MELP (derived from MDA-MB-231) and stably expressing estrogen receptor  (ER); these cell lines stably express estrogen response element (β-globin)-luciferase. Genistein, bisphenol A (BPA), 4-(tert-octyl)phenol (OP), dieldrin, and several phthalates, including benzyl butyl phthalate (BBP) and di-ethyl-2-hexyle phthalate (DEHP), were first shown to be estrogenic. These compounds induced a dose-dependent increase of VEGF secretion in MELN and MCF-7 cells; maximal effect was observed at 1–10 µM non-cytotoxic concentrations and was inhibited by the antiestrogen ICI 182 780. VEGF increase was not observed in ER-negative MDA-MB-231 cells. Most substances increased VEGF transcript levels in MELN cells. In contrast, -hexachlorocyclohexane, vinclozolin, and the phthalates (mono-n-butyl ester phthalic acid, di-isononyle phthalate, and di-isodecyle phthalate) were ineffective on both VEGF secretion and estrogenic luciferase induction in these cell lines. Specific kinase inhibitors PD98059, SB203580, or LY294002 suppressed the xenoestrogen-induced VEGF response, suggesting activation of MEK, p38 kinase, and phosphatidylinositol-3-kinase pathways. Our in vitro results show for the first time that genistein and xenoestrogens (BPA, OP, dieldrin, BBP, and DEHP at high concentrations) up-regulate VEGF expression in MELN cells by an ER-dependent mechanism. Since VEGF increases capillary permeability and breast tumor angiogenesis in vivo, the physiological relevance of these findings is discussed. http://joe.endocrinology-journals.org/cgi/content/abstract/196/2/399	topic_bc
78133	9	356084	6	NULL	NULL	NULL	NULL	dieldrin	Chemical		increases					VEGF	GP	secretion of			NULL	MELN cells	NULL	NULL	NULL	NULL	NULL	NULL	nvironmental chemicals may affect human health by disrupting endocrine function. Their possible role in the mammary gland and breast tumors is still unknown. Previous studies have demonstrated that vascular endothelial growth factor (VEGF), a key factor in angiogenesis and tumor progression, is an estrogen-regulated gene. We analyzed whether VEGF expression is regulated by different xenoestrogens in several breast cancer cells, MELN (derived from MCF-7) and MELP (derived from MDA-MB-231) and stably expressing estrogen receptor  (ER); these cell lines stably express estrogen response element (β-globin)-luciferase. Genistein, bisphenol A (BPA), 4-(tert-octyl)phenol (OP), dieldrin, and several phthalates, including benzyl butyl phthalate (BBP) and di-ethyl-2-hexyle phthalate (DEHP), were first shown to be estrogenic. These compounds induced a dose-dependent increase of VEGF secretion in MELN and MCF-7 cells; maximal effect was observed at 1–10 µM non-cytotoxic concentrations and was inhibited by the antiestrogen ICI 182 780. VEGF increase was not observed in ER-negative MDA-MB-231 cells. Most substances increased VEGF transcript levels in MELN cells. In contrast, -hexachlorocyclohexane, vinclozolin, and the phthalates (mono-n-butyl ester phthalic acid, di-isononyle phthalate, and di-isodecyle phthalate) were ineffective on both VEGF secretion and estrogenic luciferase induction in these cell lines. Specific kinase inhibitors PD98059, SB203580, or LY294002 suppressed the xenoestrogen-induced VEGF response, suggesting activation of MEK, p38 kinase, and phosphatidylinositol-3-kinase pathways. Our in vitro results show for the first time that genistein and xenoestrogens (BPA, OP, dieldrin, BBP, and DEHP at high concentrations) up-regulate VEGF expression in MELN cells by an ER-dependent mechanism. Since VEGF increases capillary permeability and breast tumor angiogenesis in vivo, the physiological relevance of these findings is discussed. http://joe.endocrinology-journals.org/cgi/content/abstract/196/2/399	topic_bc
78134	10	356084	6	NULL	NULL	NULL	NULL	BBP	Chemical		increases					VEGF	GP	secretion of			NULL	MELN cells	NULL	NULL	NULL	NULL	NULL	NULL	nvironmental chemicals may affect human health by disrupting endocrine function. Their possible role in the mammary gland and breast tumors is still unknown. Previous studies have demonstrated that vascular endothelial growth factor (VEGF), a key factor in angiogenesis and tumor progression, is an estrogen-regulated gene. We analyzed whether VEGF expression is regulated by different xenoestrogens in several breast cancer cells, MELN (derived from MCF-7) and MELP (derived from MDA-MB-231) and stably expressing estrogen receptor  (ER); these cell lines stably express estrogen response element (β-globin)-luciferase. Genistein, bisphenol A (BPA), 4-(tert-octyl)phenol (OP), dieldrin, and several phthalates, including benzyl butyl phthalate (BBP) and di-ethyl-2-hexyle phthalate (DEHP), were first shown to be estrogenic. These compounds induced a dose-dependent increase of VEGF secretion in MELN and MCF-7 cells; maximal effect was observed at 1–10 µM non-cytotoxic concentrations and was inhibited by the antiestrogen ICI 182 780. VEGF increase was not observed in ER-negative MDA-MB-231 cells. Most substances increased VEGF transcript levels in MELN cells. In contrast, -hexachlorocyclohexane, vinclozolin, and the phthalates (mono-n-butyl ester phthalic acid, di-isononyle phthalate, and di-isodecyle phthalate) were ineffective on both VEGF secretion and estrogenic luciferase induction in these cell lines. Specific kinase inhibitors PD98059, SB203580, or LY294002 suppressed the xenoestrogen-induced VEGF response, suggesting activation of MEK, p38 kinase, and phosphatidylinositol-3-kinase pathways. Our in vitro results show for the first time that genistein and xenoestrogens (BPA, OP, dieldrin, BBP, and DEHP at high concentrations) up-regulate VEGF expression in MELN cells by an ER-dependent mechanism. Since VEGF increases capillary permeability and breast tumor angiogenesis in vivo, the physiological relevance of these findings is discussed. http://joe.endocrinology-journals.org/cgi/content/abstract/196/2/399	topic_bc
78137	11	356084	6	NULL	NULL	0	NULL	BBP			is					benzyl butyl phthalate					NULL		0	NULL	NULL	NULL	NULL	NULL	nvironmental chemicals may affect human health by disrupting endocrine function. Their possible role in the mammary gland and breast tumors is still unknown. Previous studies have demonstrated that vascular endothelial growth factor (VEGF), a key factor in angiogenesis and tumor progression, is an estrogen-regulated gene. We analyzed whether VEGF expression is regulated by different xenoestrogens in several breast cancer cells, MELN (derived from MCF-7) and MELP (derived from MDA-MB-231) and stably expressing estrogen receptor  (ER); these cell lines stably express estrogen response element (β-globin)-luciferase. Genistein, bisphenol A (BPA), 4-(tert-octyl)phenol (OP), dieldrin, and several phthalates, including benzyl butyl phthalate (BBP) and di-ethyl-2-hexyle phthalate (DEHP), were first shown to be estrogenic. These compounds induced a dose-dependent increase of VEGF secretion in MELN and MCF-7 cells; maximal effect was observed at 1–10 µM non-cytotoxic concentrations and was inhibited by the antiestrogen ICI 182 780. VEGF increase was not observed in ER-negative MDA-MB-231 cells. Most substances increased VEGF transcript levels in MELN cells. In contrast, -hexachlorocyclohexane, vinclozolin, and the phthalates (mono-n-butyl ester phthalic acid, di-isononyle phthalate, and di-isodecyle phthalate) were ineffective on both VEGF secretion and estrogenic luciferase induction in these cell lines. Specific kinase inhibitors PD98059, SB203580, or LY294002 suppressed the xenoestrogen-induced VEGF response, suggesting activation of MEK, p38 kinase, and phosphatidylinositol-3-kinase pathways. Our in vitro results show for the first time that genistein and xenoestrogens (BPA, OP, dieldrin, BBP, and DEHP at high concentrations) up-regulate VEGF expression in MELN cells by an ER-dependent mechanism. Since VEGF increases capillary permeability and breast tumor angiogenesis in vivo, the physiological relevance of these findings is discussed. http://joe.endocrinology-journals.org/cgi/content/abstract/196/2/399	topic_bc
78140	12	356084	6	NULL	NULL	0	NULL	di-ethyl-2-hexyle phthalate	Chemical		is					DEHP	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	nvironmental chemicals may affect human health by disrupting endocrine function. Their possible role in the mammary gland and breast tumors is still unknown. Previous studies have demonstrated that vascular endothelial growth factor (VEGF), a key factor in angiogenesis and tumor progression, is an estrogen-regulated gene. We analyzed whether VEGF expression is regulated by different xenoestrogens in several breast cancer cells, MELN (derived from MCF-7) and MELP (derived from MDA-MB-231) and stably expressing estrogen receptor  (ER); these cell lines stably express estrogen response element (β-globin)-luciferase. Genistein, bisphenol A (BPA), 4-(tert-octyl)phenol (OP), dieldrin, and several phthalates, including benzyl butyl phthalate (BBP) and di-ethyl-2-hexyle phthalate (DEHP), were first shown to be estrogenic. These compounds induced a dose-dependent increase of VEGF secretion in MELN and MCF-7 cells; maximal effect was observed at 1–10 µM non-cytotoxic concentrations and was inhibited by the antiestrogen ICI 182 780. VEGF increase was not observed in ER-negative MDA-MB-231 cells. Most substances increased VEGF transcript levels in MELN cells. In contrast, -hexachlorocyclohexane, vinclozolin, and the phthalates (mono-n-butyl ester phthalic acid, di-isononyle phthalate, and di-isodecyle phthalate) were ineffective on both VEGF secretion and estrogenic luciferase induction in these cell lines. Specific kinase inhibitors PD98059, SB203580, or LY294002 suppressed the xenoestrogen-induced VEGF response, suggesting activation of MEK, p38 kinase, and phosphatidylinositol-3-kinase pathways. Our in vitro results show for the first time that genistein and xenoestrogens (BPA, OP, dieldrin, BBP, and DEHP at high concentrations) up-regulate VEGF expression in MELN cells by an ER-dependent mechanism. Since VEGF increases capillary permeability and breast tumor angiogenesis in vivo, the physiological relevance of these findings is discussed. http://joe.endocrinology-journals.org/cgi/content/abstract/196/2/399	topic_bc
78142	13	356084	6	NULL	NULL	NULL	NULL	DEHP	Chemical		increases					VEGF	GP	secretion of			NULL	MELN cells	NULL	NULL	NULL	NULL	NULL	NULL	nvironmental chemicals may affect human health by disrupting endocrine function. Their possible role in the mammary gland and breast tumors is still unknown. Previous studies have demonstrated that vascular endothelial growth factor (VEGF), a key factor in angiogenesis and tumor progression, is an estrogen-regulated gene. We analyzed whether VEGF expression is regulated by different xenoestrogens in several breast cancer cells, MELN (derived from MCF-7) and MELP (derived from MDA-MB-231) and stably expressing estrogen receptor  (ER); these cell lines stably express estrogen response element (β-globin)-luciferase. Genistein, bisphenol A (BPA), 4-(tert-octyl)phenol (OP), dieldrin, and several phthalates, including benzyl butyl phthalate (BBP) and di-ethyl-2-hexyle phthalate (DEHP), were first shown to be estrogenic. These compounds induced a dose-dependent increase of VEGF secretion in MELN and MCF-7 cells; maximal effect was observed at 1–10 µM non-cytotoxic concentrations and was inhibited by the antiestrogen ICI 182 780. VEGF increase was not observed in ER-negative MDA-MB-231 cells. Most substances increased VEGF transcript levels in MELN cells. In contrast, -hexachlorocyclohexane, vinclozolin, and the phthalates (mono-n-butyl ester phthalic acid, di-isononyle phthalate, and di-isodecyle phthalate) were ineffective on both VEGF secretion and estrogenic luciferase induction in these cell lines. Specific kinase inhibitors PD98059, SB203580, or LY294002 suppressed the xenoestrogen-induced VEGF response, suggesting activation of MEK, p38 kinase, and phosphatidylinositol-3-kinase pathways. Our in vitro results show for the first time that genistein and xenoestrogens (BPA, OP, dieldrin, BBP, and DEHP at high concentrations) up-regulate VEGF expression in MELN cells by an ER-dependent mechanism. Since VEGF increases capillary permeability and breast tumor angiogenesis in vivo, the physiological relevance of these findings is discussed. http://joe.endocrinology-journals.org/cgi/content/abstract/196/2/399	topic_bc
78144	14	356084	6	NULL	NULL	0	NULL	Genistein	Chemical		increases					VEGF	GP	secretion of			NULL	MCF-7 cells	0	NULL	NULL	NULL	NULL	NULL	nvironmental chemicals may affect human health by disrupting endocrine function. Their possible role in the mammary gland and breast tumors is still unknown. Previous studies have demonstrated that vascular endothelial growth factor (VEGF), a key factor in angiogenesis and tumor progression, is an estrogen-regulated gene. We analyzed whether VEGF expression is regulated by different xenoestrogens in several breast cancer cells, MELN (derived from MCF-7) and MELP (derived from MDA-MB-231) and stably expressing estrogen receptor  (ER); these cell lines stably express estrogen response element (β-globin)-luciferase. Genistein, bisphenol A (BPA), 4-(tert-octyl)phenol (OP), dieldrin, and several phthalates, including benzyl butyl phthalate (BBP) and di-ethyl-2-hexyle phthalate (DEHP), were first shown to be estrogenic. These compounds induced a dose-dependent increase of VEGF secretion in MELN and MCF-7 cells; maximal effect was observed at 1–10 µM non-cytotoxic concentrations and was inhibited by the antiestrogen ICI 182 780. VEGF increase was not observed in ER-negative MDA-MB-231 cells. Most substances increased VEGF transcript levels in MELN cells. In contrast, -hexachlorocyclohexane, vinclozolin, and the phthalates (mono-n-butyl ester phthalic acid, di-isononyle phthalate, and di-isodecyle phthalate) were ineffective on both VEGF secretion and estrogenic luciferase induction in these cell lines. Specific kinase inhibitors PD98059, SB203580, or LY294002 suppressed the xenoestrogen-induced VEGF response, suggesting activation of MEK, p38 kinase, and phosphatidylinositol-3-kinase pathways. Our in vitro results show for the first time that genistein and xenoestrogens (BPA, OP, dieldrin, BBP, and DEHP at high concentrations) up-regulate VEGF expression in MELN cells by an ER-dependent mechanism. Since VEGF increases capillary permeability and breast tumor angiogenesis in vivo, the physiological relevance of these findings is discussed. http://joe.endocrinology-journals.org/cgi/content/abstract/196/2/399	topic_bc
78145	15	356084	6	NULL	NULL	0	NULL	BPA	Chemical		increases					VEGF	GP	secretion of			NULL	MCF-7 cells	0	NULL	NULL	NULL	NULL	NULL	nvironmental chemicals may affect human health by disrupting endocrine function. Their possible role in the mammary gland and breast tumors is still unknown. Previous studies have demonstrated that vascular endothelial growth factor (VEGF), a key factor in angiogenesis and tumor progression, is an estrogen-regulated gene. We analyzed whether VEGF expression is regulated by different xenoestrogens in several breast cancer cells, MELN (derived from MCF-7) and MELP (derived from MDA-MB-231) and stably expressing estrogen receptor  (ER); these cell lines stably express estrogen response element (β-globin)-luciferase. Genistein, bisphenol A (BPA), 4-(tert-octyl)phenol (OP), dieldrin, and several phthalates, including benzyl butyl phthalate (BBP) and di-ethyl-2-hexyle phthalate (DEHP), were first shown to be estrogenic. These compounds induced a dose-dependent increase of VEGF secretion in MELN and MCF-7 cells; maximal effect was observed at 1–10 µM non-cytotoxic concentrations and was inhibited by the antiestrogen ICI 182 780. VEGF increase was not observed in ER-negative MDA-MB-231 cells. Most substances increased VEGF transcript levels in MELN cells. In contrast, -hexachlorocyclohexane, vinclozolin, and the phthalates (mono-n-butyl ester phthalic acid, di-isononyle phthalate, and di-isodecyle phthalate) were ineffective on both VEGF secretion and estrogenic luciferase induction in these cell lines. Specific kinase inhibitors PD98059, SB203580, or LY294002 suppressed the xenoestrogen-induced VEGF response, suggesting activation of MEK, p38 kinase, and phosphatidylinositol-3-kinase pathways. Our in vitro results show for the first time that genistein and xenoestrogens (BPA, OP, dieldrin, BBP, and DEHP at high concentrations) up-regulate VEGF expression in MELN cells by an ER-dependent mechanism. Since VEGF increases capillary permeability and breast tumor angiogenesis in vivo, the physiological relevance of these findings is discussed. http://joe.endocrinology-journals.org/cgi/content/abstract/196/2/399	topic_bc
78146	16	356084	6	NULL	NULL	0	NULL	OP	Chemical		increases					VEGF	GP	secretion of			NULL	MCF-7 cells	0	NULL	NULL	NULL	NULL	NULL	nvironmental chemicals may affect human health by disrupting endocrine function. Their possible role in the mammary gland and breast tumors is still unknown. Previous studies have demonstrated that vascular endothelial growth factor (VEGF), a key factor in angiogenesis and tumor progression, is an estrogen-regulated gene. We analyzed whether VEGF expression is regulated by different xenoestrogens in several breast cancer cells, MELN (derived from MCF-7) and MELP (derived from MDA-MB-231) and stably expressing estrogen receptor  (ER); these cell lines stably express estrogen response element (β-globin)-luciferase. Genistein, bisphenol A (BPA), 4-(tert-octyl)phenol (OP), dieldrin, and several phthalates, including benzyl butyl phthalate (BBP) and di-ethyl-2-hexyle phthalate (DEHP), were first shown to be estrogenic. These compounds induced a dose-dependent increase of VEGF secretion in MELN and MCF-7 cells; maximal effect was observed at 1–10 µM non-cytotoxic concentrations and was inhibited by the antiestrogen ICI 182 780. VEGF increase was not observed in ER-negative MDA-MB-231 cells. Most substances increased VEGF transcript levels in MELN cells. In contrast, -hexachlorocyclohexane, vinclozolin, and the phthalates (mono-n-butyl ester phthalic acid, di-isononyle phthalate, and di-isodecyle phthalate) were ineffective on both VEGF secretion and estrogenic luciferase induction in these cell lines. Specific kinase inhibitors PD98059, SB203580, or LY294002 suppressed the xenoestrogen-induced VEGF response, suggesting activation of MEK, p38 kinase, and phosphatidylinositol-3-kinase pathways. Our in vitro results show for the first time that genistein and xenoestrogens (BPA, OP, dieldrin, BBP, and DEHP at high concentrations) up-regulate VEGF expression in MELN cells by an ER-dependent mechanism. Since VEGF increases capillary permeability and breast tumor angiogenesis in vivo, the physiological relevance of these findings is discussed. http://joe.endocrinology-journals.org/cgi/content/abstract/196/2/399	topic_bc
78147	17	356084	6	NULL	NULL	0	NULL	dieldrin	Chemical		increases					VEGF	GP	secretion of			NULL	MCF-7 cells	0	NULL	NULL	NULL	NULL	NULL	nvironmental chemicals may affect human health by disrupting endocrine function. Their possible role in the mammary gland and breast tumors is still unknown. Previous studies have demonstrated that vascular endothelial growth factor (VEGF), a key factor in angiogenesis and tumor progression, is an estrogen-regulated gene. We analyzed whether VEGF expression is regulated by different xenoestrogens in several breast cancer cells, MELN (derived from MCF-7) and MELP (derived from MDA-MB-231) and stably expressing estrogen receptor  (ER); these cell lines stably express estrogen response element (β-globin)-luciferase. Genistein, bisphenol A (BPA), 4-(tert-octyl)phenol (OP), dieldrin, and several phthalates, including benzyl butyl phthalate (BBP) and di-ethyl-2-hexyle phthalate (DEHP), were first shown to be estrogenic. These compounds induced a dose-dependent increase of VEGF secretion in MELN and MCF-7 cells; maximal effect was observed at 1–10 µM non-cytotoxic concentrations and was inhibited by the antiestrogen ICI 182 780. VEGF increase was not observed in ER-negative MDA-MB-231 cells. Most substances increased VEGF transcript levels in MELN cells. In contrast, -hexachlorocyclohexane, vinclozolin, and the phthalates (mono-n-butyl ester phthalic acid, di-isononyle phthalate, and di-isodecyle phthalate) were ineffective on both VEGF secretion and estrogenic luciferase induction in these cell lines. Specific kinase inhibitors PD98059, SB203580, or LY294002 suppressed the xenoestrogen-induced VEGF response, suggesting activation of MEK, p38 kinase, and phosphatidylinositol-3-kinase pathways. Our in vitro results show for the first time that genistein and xenoestrogens (BPA, OP, dieldrin, BBP, and DEHP at high concentrations) up-regulate VEGF expression in MELN cells by an ER-dependent mechanism. Since VEGF increases capillary permeability and breast tumor angiogenesis in vivo, the physiological relevance of these findings is discussed. http://joe.endocrinology-journals.org/cgi/content/abstract/196/2/399	topic_bc
78148	18	356084	6	NULL	NULL	NULL	NULL	DEHP	Chemical		increases					VEGF	GP	secretion of			NULL	MCF-7 cells	NULL	NULL	NULL	NULL	NULL	NULL	nvironmental chemicals may affect human health by disrupting endocrine function. Their possible role in the mammary gland and breast tumors is still unknown. Previous studies have demonstrated that vascular endothelial growth factor (VEGF), a key factor in angiogenesis and tumor progression, is an estrogen-regulated gene. We analyzed whether VEGF expression is regulated by different xenoestrogens in several breast cancer cells, MELN (derived from MCF-7) and MELP (derived from MDA-MB-231) and stably expressing estrogen receptor  (ER); these cell lines stably express estrogen response element (β-globin)-luciferase. Genistein, bisphenol A (BPA), 4-(tert-octyl)phenol (OP), dieldrin, and several phthalates, including benzyl butyl phthalate (BBP) and di-ethyl-2-hexyle phthalate (DEHP), were first shown to be estrogenic. These compounds induced a dose-dependent increase of VEGF secretion in MELN and MCF-7 cells; maximal effect was observed at 1–10 µM non-cytotoxic concentrations and was inhibited by the antiestrogen ICI 182 780. VEGF increase was not observed in ER-negative MDA-MB-231 cells. Most substances increased VEGF transcript levels in MELN cells. In contrast, -hexachlorocyclohexane, vinclozolin, and the phthalates (mono-n-butyl ester phthalic acid, di-isononyle phthalate, and di-isodecyle phthalate) were ineffective on both VEGF secretion and estrogenic luciferase induction in these cell lines. Specific kinase inhibitors PD98059, SB203580, or LY294002 suppressed the xenoestrogen-induced VEGF response, suggesting activation of MEK, p38 kinase, and phosphatidylinositol-3-kinase pathways. Our in vitro results show for the first time that genistein and xenoestrogens (BPA, OP, dieldrin, BBP, and DEHP at high concentrations) up-regulate VEGF expression in MELN cells by an ER-dependent mechanism. Since VEGF increases capillary permeability and breast tumor angiogenesis in vivo, the physiological relevance of these findings is discussed. http://joe.endocrinology-journals.org/cgi/content/abstract/196/2/399	topic_bc
78155	19	356084	6	NULL	NULL	0	NULL	BBP	Chemical		increases					VEGF	GP	secretion of			NULL		0	NULL	NULL	NULL	NULL	NULL	nvironmental chemicals may affect human health by disrupting endocrine function. Their possible role in the mammary gland and breast tumors is still unknown. Previous studies have demonstrated that vascular endothelial growth factor (VEGF), a key factor in angiogenesis and tumor progression, is an estrogen-regulated gene. We analyzed whether VEGF expression is regulated by different xenoestrogens in several breast cancer cells, MELN (derived from MCF-7) and MELP (derived from MDA-MB-231) and stably expressing estrogen receptor  (ER); these cell lines stably express estrogen response element (β-globin)-luciferase. Genistein, bisphenol A (BPA), 4-(tert-octyl)phenol (OP), dieldrin, and several phthalates, including benzyl butyl phthalate (BBP) and di-ethyl-2-hexyle phthalate (DEHP), were first shown to be estrogenic. These compounds induced a dose-dependent increase of VEGF secretion in MELN and MCF-7 cells; maximal effect was observed at 1–10 µM non-cytotoxic concentrations and was inhibited by the antiestrogen ICI 182 780. VEGF increase was not observed in ER-negative MDA-MB-231 cells. Most substances increased VEGF transcript levels in MELN cells. In contrast, -hexachlorocyclohexane, vinclozolin, and the phthalates (mono-n-butyl ester phthalic acid, di-isononyle phthalate, and di-isodecyle phthalate) were ineffective on both VEGF secretion and estrogenic luciferase induction in these cell lines. Specific kinase inhibitors PD98059, SB203580, or LY294002 suppressed the xenoestrogen-induced VEGF response, suggesting activation of MEK, p38 kinase, and phosphatidylinositol-3-kinase pathways. Our in vitro results show for the first time that genistein and xenoestrogens (BPA, OP, dieldrin, BBP, and DEHP at high concentrations) up-regulate VEGF expression in MELN cells by an ER-dependent mechanism. Since VEGF increases capillary permeability and breast tumor angiogenesis in vivo, the physiological relevance of these findings is discussed. http://joe.endocrinology-journals.org/cgi/content/abstract/196/2/399	topic_bc
78157	20	356084	6	NULL	NULL	0	NULL	BPA	Chemical		is a type of					xenoestrogen	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	nvironmental chemicals may affect human health by disrupting endocrine function. Their possible role in the mammary gland and breast tumors is still unknown. Previous studies have demonstrated that vascular endothelial growth factor (VEGF), a key factor in angiogenesis and tumor progression, is an estrogen-regulated gene. We analyzed whether VEGF expression is regulated by different xenoestrogens in several breast cancer cells, MELN (derived from MCF-7) and MELP (derived from MDA-MB-231) and stably expressing estrogen receptor  (ER); these cell lines stably express estrogen response element (β-globin)-luciferase. Genistein, bisphenol A (BPA), 4-(tert-octyl)phenol (OP), dieldrin, and several phthalates, including benzyl butyl phthalate (BBP) and di-ethyl-2-hexyle phthalate (DEHP), were first shown to be estrogenic. These compounds induced a dose-dependent increase of VEGF secretion in MELN and MCF-7 cells; maximal effect was observed at 1–10 µM non-cytotoxic concentrations and was inhibited by the antiestrogen ICI 182 780. VEGF increase was not observed in ER-negative MDA-MB-231 cells. Most substances increased VEGF transcript levels in MELN cells. In contrast, -hexachlorocyclohexane, vinclozolin, and the phthalates (mono-n-butyl ester phthalic acid, di-isononyle phthalate, and di-isodecyle phthalate) were ineffective on both VEGF secretion and estrogenic luciferase induction in these cell lines. Specific kinase inhibitors PD98059, SB203580, or LY294002 suppressed the xenoestrogen-induced VEGF response, suggesting activation of MEK, p38 kinase, and phosphatidylinositol-3-kinase pathways. Our in vitro results show for the first time that genistein and xenoestrogens (BPA, OP, dieldrin, BBP, and DEHP at high concentrations) up-regulate VEGF expression in MELN cells by an ER-dependent mechanism. Since VEGF increases capillary permeability and breast tumor angiogenesis in vivo, the physiological relevance of these findings is discussed. http://joe.endocrinology-journals.org/cgi/content/abstract/196/2/399	topic_bc
78160	21	356084	6	NULL	NULL	0	NULL	OP	Chemical		is a type of					xenoestrogen	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	nvironmental chemicals may affect human health by disrupting endocrine function. Their possible role in the mammary gland and breast tumors is still unknown. Previous studies have demonstrated that vascular endothelial growth factor (VEGF), a key factor in angiogenesis and tumor progression, is an estrogen-regulated gene. We analyzed whether VEGF expression is regulated by different xenoestrogens in several breast cancer cells, MELN (derived from MCF-7) and MELP (derived from MDA-MB-231) and stably expressing estrogen receptor  (ER); these cell lines stably express estrogen response element (β-globin)-luciferase. Genistein, bisphenol A (BPA), 4-(tert-octyl)phenol (OP), dieldrin, and several phthalates, including benzyl butyl phthalate (BBP) and di-ethyl-2-hexyle phthalate (DEHP), were first shown to be estrogenic. These compounds induced a dose-dependent increase of VEGF secretion in MELN and MCF-7 cells; maximal effect was observed at 1–10 µM non-cytotoxic concentrations and was inhibited by the antiestrogen ICI 182 780. VEGF increase was not observed in ER-negative MDA-MB-231 cells. Most substances increased VEGF transcript levels in MELN cells. In contrast, -hexachlorocyclohexane, vinclozolin, and the phthalates (mono-n-butyl ester phthalic acid, di-isononyle phthalate, and di-isodecyle phthalate) were ineffective on both VEGF secretion and estrogenic luciferase induction in these cell lines. Specific kinase inhibitors PD98059, SB203580, or LY294002 suppressed the xenoestrogen-induced VEGF response, suggesting activation of MEK, p38 kinase, and phosphatidylinositol-3-kinase pathways. Our in vitro results show for the first time that genistein and xenoestrogens (BPA, OP, dieldrin, BBP, and DEHP at high concentrations) up-regulate VEGF expression in MELN cells by an ER-dependent mechanism. Since VEGF increases capillary permeability and breast tumor angiogenesis in vivo, the physiological relevance of these findings is discussed. http://joe.endocrinology-journals.org/cgi/content/abstract/196/2/399	topic_bc
78161	22	356084	6	NULL	NULL	0	NULL	dieldrin	Chemical		is a type of					xenoestrogen	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	nvironmental chemicals may affect human health by disrupting endocrine function. Their possible role in the mammary gland and breast tumors is still unknown. Previous studies have demonstrated that vascular endothelial growth factor (VEGF), a key factor in angiogenesis and tumor progression, is an estrogen-regulated gene. We analyzed whether VEGF expression is regulated by different xenoestrogens in several breast cancer cells, MELN (derived from MCF-7) and MELP (derived from MDA-MB-231) and stably expressing estrogen receptor  (ER); these cell lines stably express estrogen response element (β-globin)-luciferase. Genistein, bisphenol A (BPA), 4-(tert-octyl)phenol (OP), dieldrin, and several phthalates, including benzyl butyl phthalate (BBP) and di-ethyl-2-hexyle phthalate (DEHP), were first shown to be estrogenic. These compounds induced a dose-dependent increase of VEGF secretion in MELN and MCF-7 cells; maximal effect was observed at 1–10 µM non-cytotoxic concentrations and was inhibited by the antiestrogen ICI 182 780. VEGF increase was not observed in ER-negative MDA-MB-231 cells. Most substances increased VEGF transcript levels in MELN cells. In contrast, -hexachlorocyclohexane, vinclozolin, and the phthalates (mono-n-butyl ester phthalic acid, di-isononyle phthalate, and di-isodecyle phthalate) were ineffective on both VEGF secretion and estrogenic luciferase induction in these cell lines. Specific kinase inhibitors PD98059, SB203580, or LY294002 suppressed the xenoestrogen-induced VEGF response, suggesting activation of MEK, p38 kinase, and phosphatidylinositol-3-kinase pathways. Our in vitro results show for the first time that genistein and xenoestrogens (BPA, OP, dieldrin, BBP, and DEHP at high concentrations) up-regulate VEGF expression in MELN cells by an ER-dependent mechanism. Since VEGF increases capillary permeability and breast tumor angiogenesis in vivo, the physiological relevance of these findings is discussed. http://joe.endocrinology-journals.org/cgi/content/abstract/196/2/399	topic_bc
78162	23	356084	6	NULL	NULL	0	NULL	BBP	Chemical		is a type of					xenoestrogen	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	nvironmental chemicals may affect human health by disrupting endocrine function. Their possible role in the mammary gland and breast tumors is still unknown. Previous studies have demonstrated that vascular endothelial growth factor (VEGF), a key factor in angiogenesis and tumor progression, is an estrogen-regulated gene. We analyzed whether VEGF expression is regulated by different xenoestrogens in several breast cancer cells, MELN (derived from MCF-7) and MELP (derived from MDA-MB-231) and stably expressing estrogen receptor  (ER); these cell lines stably express estrogen response element (β-globin)-luciferase. Genistein, bisphenol A (BPA), 4-(tert-octyl)phenol (OP), dieldrin, and several phthalates, including benzyl butyl phthalate (BBP) and di-ethyl-2-hexyle phthalate (DEHP), were first shown to be estrogenic. These compounds induced a dose-dependent increase of VEGF secretion in MELN and MCF-7 cells; maximal effect was observed at 1–10 µM non-cytotoxic concentrations and was inhibited by the antiestrogen ICI 182 780. VEGF increase was not observed in ER-negative MDA-MB-231 cells. Most substances increased VEGF transcript levels in MELN cells. In contrast, -hexachlorocyclohexane, vinclozolin, and the phthalates (mono-n-butyl ester phthalic acid, di-isononyle phthalate, and di-isodecyle phthalate) were ineffective on both VEGF secretion and estrogenic luciferase induction in these cell lines. Specific kinase inhibitors PD98059, SB203580, or LY294002 suppressed the xenoestrogen-induced VEGF response, suggesting activation of MEK, p38 kinase, and phosphatidylinositol-3-kinase pathways. Our in vitro results show for the first time that genistein and xenoestrogens (BPA, OP, dieldrin, BBP, and DEHP at high concentrations) up-regulate VEGF expression in MELN cells by an ER-dependent mechanism. Since VEGF increases capillary permeability and breast tumor angiogenesis in vivo, the physiological relevance of these findings is discussed. http://joe.endocrinology-journals.org/cgi/content/abstract/196/2/399	topic_bc
78163	24	356084	6	NULL	NULL	0	NULL	DEHP	Chemical		is a type of					xenoestrogen	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	nvironmental chemicals may affect human health by disrupting endocrine function. Their possible role in the mammary gland and breast tumors is still unknown. Previous studies have demonstrated that vascular endothelial growth factor (VEGF), a key factor in angiogenesis and tumor progression, is an estrogen-regulated gene. We analyzed whether VEGF expression is regulated by different xenoestrogens in several breast cancer cells, MELN (derived from MCF-7) and MELP (derived from MDA-MB-231) and stably expressing estrogen receptor  (ER); these cell lines stably express estrogen response element (β-globin)-luciferase. Genistein, bisphenol A (BPA), 4-(tert-octyl)phenol (OP), dieldrin, and several phthalates, including benzyl butyl phthalate (BBP) and di-ethyl-2-hexyle phthalate (DEHP), were first shown to be estrogenic. These compounds induced a dose-dependent increase of VEGF secretion in MELN and MCF-7 cells; maximal effect was observed at 1–10 µM non-cytotoxic concentrations and was inhibited by the antiestrogen ICI 182 780. VEGF increase was not observed in ER-negative MDA-MB-231 cells. Most substances increased VEGF transcript levels in MELN cells. In contrast, -hexachlorocyclohexane, vinclozolin, and the phthalates (mono-n-butyl ester phthalic acid, di-isononyle phthalate, and di-isodecyle phthalate) were ineffective on both VEGF secretion and estrogenic luciferase induction in these cell lines. Specific kinase inhibitors PD98059, SB203580, or LY294002 suppressed the xenoestrogen-induced VEGF response, suggesting activation of MEK, p38 kinase, and phosphatidylinositol-3-kinase pathways. Our in vitro results show for the first time that genistein and xenoestrogens (BPA, OP, dieldrin, BBP, and DEHP at high concentrations) up-regulate VEGF expression in MELN cells by an ER-dependent mechanism. Since VEGF increases capillary permeability and breast tumor angiogenesis in vivo, the physiological relevance of these findings is discussed. http://joe.endocrinology-journals.org/cgi/content/abstract/196/2/399	topic_bc
78164	25	356084	6	NULL	NULL	NULL	NULL	VEGF	GP		increases					capillary	OrganismPart	permeability of 			NULL	in vivo	NULL	NULL	NULL	NULL	NULL	NULL	nvironmental chemicals may affect human health by disrupting endocrine function. Their possible role in the mammary gland and breast tumors is still unknown. Previous studies have demonstrated that vascular endothelial growth factor (VEGF), a key factor in angiogenesis and tumor progression, is an estrogen-regulated gene. We analyzed whether VEGF expression is regulated by different xenoestrogens in several breast cancer cells, MELN (derived from MCF-7) and MELP (derived from MDA-MB-231) and stably expressing estrogen receptor  (ER); these cell lines stably express estrogen response element (β-globin)-luciferase. Genistein, bisphenol A (BPA), 4-(tert-octyl)phenol (OP), dieldrin, and several phthalates, including benzyl butyl phthalate (BBP) and di-ethyl-2-hexyle phthalate (DEHP), were first shown to be estrogenic. These compounds induced a dose-dependent increase of VEGF secretion in MELN and MCF-7 cells; maximal effect was observed at 1–10 µM non-cytotoxic concentrations and was inhibited by the antiestrogen ICI 182 780. VEGF increase was not observed in ER-negative MDA-MB-231 cells. Most substances increased VEGF transcript levels in MELN cells. In contrast, -hexachlorocyclohexane, vinclozolin, and the phthalates (mono-n-butyl ester phthalic acid, di-isononyle phthalate, and di-isodecyle phthalate) were ineffective on both VEGF secretion and estrogenic luciferase induction in these cell lines. Specific kinase inhibitors PD98059, SB203580, or LY294002 suppressed the xenoestrogen-induced VEGF response, suggesting activation of MEK, p38 kinase, and phosphatidylinositol-3-kinase pathways. Our in vitro results show for the first time that genistein and xenoestrogens (BPA, OP, dieldrin, BBP, and DEHP at high concentrations) up-regulate VEGF expression in MELN cells by an ER-dependent mechanism. Since VEGF increases capillary permeability and breast tumor angiogenesis in vivo, the physiological relevance of these findings is discussed. http://joe.endocrinology-journals.org/cgi/content/abstract/196/2/399	topic_bc
78165	26	356084	6	NULL	NULL	NULL	NULL	VEGF	GP		increases					angiogenesis	process				NULL	in vivo	NULL	NULL	NULL	NULL	NULL	NULL	nvironmental chemicals may affect human health by disrupting endocrine function. Their possible role in the mammary gland and breast tumors is still unknown. Previous studies have demonstrated that vascular endothelial growth factor (VEGF), a key factor in angiogenesis and tumor progression, is an estrogen-regulated gene. We analyzed whether VEGF expression is regulated by different xenoestrogens in several breast cancer cells, MELN (derived from MCF-7) and MELP (derived from MDA-MB-231) and stably expressing estrogen receptor  (ER); these cell lines stably express estrogen response element (β-globin)-luciferase. Genistein, bisphenol A (BPA), 4-(tert-octyl)phenol (OP), dieldrin, and several phthalates, including benzyl butyl phthalate (BBP) and di-ethyl-2-hexyle phthalate (DEHP), were first shown to be estrogenic. These compounds induced a dose-dependent increase of VEGF secretion in MELN and MCF-7 cells; maximal effect was observed at 1–10 µM non-cytotoxic concentrations and was inhibited by the antiestrogen ICI 182 780. VEGF increase was not observed in ER-negative MDA-MB-231 cells. Most substances increased VEGF transcript levels in MELN cells. In contrast, -hexachlorocyclohexane, vinclozolin, and the phthalates (mono-n-butyl ester phthalic acid, di-isononyle phthalate, and di-isodecyle phthalate) were ineffective on both VEGF secretion and estrogenic luciferase induction in these cell lines. Specific kinase inhibitors PD98059, SB203580, or LY294002 suppressed the xenoestrogen-induced VEGF response, suggesting activation of MEK, p38 kinase, and phosphatidylinositol-3-kinase pathways. Our in vitro results show for the first time that genistein and xenoestrogens (BPA, OP, dieldrin, BBP, and DEHP at high concentrations) up-regulate VEGF expression in MELN cells by an ER-dependent mechanism. Since VEGF increases capillary permeability and breast tumor angiogenesis in vivo, the physiological relevance of these findings is discussed. http://joe.endocrinology-journals.org/cgi/content/abstract/196/2/399	topic_bc
78090	1	356085	6	NULL	NULL	0	NULL	estrogen	Chemical	deprivation of	causes					Breast cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Deprivation of estrogen causes breast tumors in women to adapt and develop enhanced sensitivity to this steroid. Accordingly, women relapsing after treatment with oophorectomy, which substantially lowers estradiol for a prolonged period, respond secondarily to aromatase inhibitors with tumor regression. We have utilized in vitro and in vivo model systems to examine the biologic processes whereby Long Term Estradiol Deprivation (LTED) causes cells to adapts and develop hypersensitivity to estradiol. Several mechanisms are associated with this response including up-regulation of ERα and the MAP kinase, PI-3-kinase and mTOR growth factor pathways. ERα is 4–10 fold up-regulated as a result of demethylation of its C promoter, This nuclear receptor then co-opts a classical growth factor pathway using SHC, Grb-2 and Sos. This induces rapid nongenomic effects which are enhanced in LTED cells. The molecules involved in the nongenomic signaling process have been identified. Estradiol binds to cell membrance-associated ERα which physically associates with the adaptor protein SHC and induces its phosphorylation. In turn, SHC binds Grb-2 and Sos which results in the rapid activation of MAP kinase. These nongenomic effects of estradiol produce biologic effects as evidenced by Elk-1 activation and by morphologic changes in cell membrances. Additional effects include activation of the PI-3-kinase and mTOR pathways through estradiol-induced binding of ERα to the IGF-1 and EGF receptors. A major question is how ERα locates in the plasma membrance since it does not contain an inherent membrance localization signal. We have provided evidence that the IGF-1 receptor serves as an anchor for ERα in the plasma membrane. Estradiol causes phosphorylation of the adaptor protein, SHC and the IGF-1 receptor itself. SHC, after binding to ERα, serves as the “glue” which tethers ERα to SHC binding sites on the activated IFG-1 receptors. Use of siRNA methodology to knock down SHC allows the conclusion that SHC is needed for ERα to localize in the plasma membrane.	topic_bc
78091	2	356085	6	NULL	NULL	0	NULL	oophorectomy	MedicalProcedure		is used for					Breast cancer	MedicalFinding	treatment of 			NULL		0	NULL	NULL	NULL	NULL	NULL	Deprivation of estrogen causes breast tumors in women to adapt and develop enhanced sensitivity to this steroid. Accordingly, women relapsing after treatment with oophorectomy, which substantially lowers estradiol for a prolonged period, respond secondarily to aromatase inhibitors with tumor regression. We have utilized in vitro and in vivo model systems to examine the biologic processes whereby Long Term Estradiol Deprivation (LTED) causes cells to adapts and develop hypersensitivity to estradiol. Several mechanisms are associated with this response including up-regulation of ERα and the MAP kinase, PI-3-kinase and mTOR growth factor pathways. ERα is 4–10 fold up-regulated as a result of demethylation of its C promoter, This nuclear receptor then co-opts a classical growth factor pathway using SHC, Grb-2 and Sos. This induces rapid nongenomic effects which are enhanced in LTED cells. The molecules involved in the nongenomic signaling process have been identified. Estradiol binds to cell membrance-associated ERα which physically associates with the adaptor protein SHC and induces its phosphorylation. In turn, SHC binds Grb-2 and Sos which results in the rapid activation of MAP kinase. These nongenomic effects of estradiol produce biologic effects as evidenced by Elk-1 activation and by morphologic changes in cell membrances. Additional effects include activation of the PI-3-kinase and mTOR pathways through estradiol-induced binding of ERα to the IGF-1 and EGF receptors. A major question is how ERα locates in the plasma membrance since it does not contain an inherent membrance localization signal. We have provided evidence that the IGF-1 receptor serves as an anchor for ERα in the plasma membrane. Estradiol causes phosphorylation of the adaptor protein, SHC and the IGF-1 receptor itself. SHC, after binding to ERα, serves as the “glue” which tethers ERα to SHC binding sites on the activated IFG-1 receptors. Use of siRNA methodology to knock down SHC allows the conclusion that SHC is needed for ERα to localize in the plasma membrane.	topic_bc
78092	3	356085	6	NULL	NULL	0	NULL	oophorectomy	MedicalProcedure		lowers					estradiol	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Deprivation of estrogen causes breast tumors in women to adapt and develop enhanced sensitivity to this steroid. Accordingly, women relapsing after treatment with oophorectomy, which substantially lowers estradiol for a prolonged period, respond secondarily to aromatase inhibitors with tumor regression. We have utilized in vitro and in vivo model systems to examine the biologic processes whereby Long Term Estradiol Deprivation (LTED) causes cells to adapts and develop hypersensitivity to estradiol. Several mechanisms are associated with this response including up-regulation of ERα and the MAP kinase, PI-3-kinase and mTOR growth factor pathways. ERα is 4–10 fold up-regulated as a result of demethylation of its C promoter, This nuclear receptor then co-opts a classical growth factor pathway using SHC, Grb-2 and Sos. This induces rapid nongenomic effects which are enhanced in LTED cells. The molecules involved in the nongenomic signaling process have been identified. Estradiol binds to cell membrance-associated ERα which physically associates with the adaptor protein SHC and induces its phosphorylation. In turn, SHC binds Grb-2 and Sos which results in the rapid activation of MAP kinase. These nongenomic effects of estradiol produce biologic effects as evidenced by Elk-1 activation and by morphologic changes in cell membrances. Additional effects include activation of the PI-3-kinase and mTOR pathways through estradiol-induced binding of ERα to the IGF-1 and EGF receptors. A major question is how ERα locates in the plasma membrance since it does not contain an inherent membrance localization signal. We have provided evidence that the IGF-1 receptor serves as an anchor for ERα in the plasma membrane. Estradiol causes phosphorylation of the adaptor protein, SHC and the IGF-1 receptor itself. SHC, after binding to ERα, serves as the “glue” which tethers ERα to SHC binding sites on the activated IFG-1 receptors. Use of siRNA methodology to knock down SHC allows the conclusion that SHC is needed for ERα to localize in the plasma membrane.	topic_bc
78093	4	356085	6	NULL	NULL	0	NULL	LTED	process		is					Long Term Estradiol Deprivation	process				NULL		0	NULL	NULL	NULL	NULL	NULL	Deprivation of estrogen causes breast tumors in women to adapt and develop enhanced sensitivity to this steroid. Accordingly, women relapsing after treatment with oophorectomy, which substantially lowers estradiol for a prolonged period, respond secondarily to aromatase inhibitors with tumor regression. We have utilized in vitro and in vivo model systems to examine the biologic processes whereby Long Term Estradiol Deprivation (LTED) causes cells to adapts and develop hypersensitivity to estradiol. Several mechanisms are associated with this response including up-regulation of ERα and the MAP kinase, PI-3-kinase and mTOR growth factor pathways. ERα is 4–10 fold up-regulated as a result of demethylation of its C promoter, This nuclear receptor then co-opts a classical growth factor pathway using SHC, Grb-2 and Sos. This induces rapid nongenomic effects which are enhanced in LTED cells. The molecules involved in the nongenomic signaling process have been identified. Estradiol binds to cell membrance-associated ERα which physically associates with the adaptor protein SHC and induces its phosphorylation. In turn, SHC binds Grb-2 and Sos which results in the rapid activation of MAP kinase. These nongenomic effects of estradiol produce biologic effects as evidenced by Elk-1 activation and by morphologic changes in cell membrances. Additional effects include activation of the PI-3-kinase and mTOR pathways through estradiol-induced binding of ERα to the IGF-1 and EGF receptors. A major question is how ERα locates in the plasma membrance since it does not contain an inherent membrance localization signal. We have provided evidence that the IGF-1 receptor serves as an anchor for ERα in the plasma membrane. Estradiol causes phosphorylation of the adaptor protein, SHC and the IGF-1 receptor itself. SHC, after binding to ERα, serves as the “glue” which tethers ERα to SHC binding sites on the activated IFG-1 receptors. Use of siRNA methodology to knock down SHC allows the conclusion that SHC is needed for ERα to localize in the plasma membrane.	topic_bc
78094	5	356085	6	NULL	NULL	0	NULL	LTED	process		causes					estradiol	Chemical	hypersensitivity to			NULL		0	NULL	NULL	NULL	NULL	NULL	Deprivation of estrogen causes breast tumors in women to adapt and develop enhanced sensitivity to this steroid. Accordingly, women relapsing after treatment with oophorectomy, which substantially lowers estradiol for a prolonged period, respond secondarily to aromatase inhibitors with tumor regression. We have utilized in vitro and in vivo model systems to examine the biologic processes whereby Long Term Estradiol Deprivation (LTED) causes cells to adapts and develop hypersensitivity to estradiol. Several mechanisms are associated with this response including up-regulation of ERα and the MAP kinase, PI-3-kinase and mTOR growth factor pathways. ERα is 4–10 fold up-regulated as a result of demethylation of its C promoter, This nuclear receptor then co-opts a classical growth factor pathway using SHC, Grb-2 and Sos. This induces rapid nongenomic effects which are enhanced in LTED cells. The molecules involved in the nongenomic signaling process have been identified. Estradiol binds to cell membrance-associated ERα which physically associates with the adaptor protein SHC and induces its phosphorylation. In turn, SHC binds Grb-2 and Sos which results in the rapid activation of MAP kinase. These nongenomic effects of estradiol produce biologic effects as evidenced by Elk-1 activation and by morphologic changes in cell membrances. Additional effects include activation of the PI-3-kinase and mTOR pathways through estradiol-induced binding of ERα to the IGF-1 and EGF receptors. A major question is how ERα locates in the plasma membrance since it does not contain an inherent membrance localization signal. We have provided evidence that the IGF-1 receptor serves as an anchor for ERα in the plasma membrane. Estradiol causes phosphorylation of the adaptor protein, SHC and the IGF-1 receptor itself. SHC, after binding to ERα, serves as the “glue” which tethers ERα to SHC binding sites on the activated IFG-1 receptors. Use of siRNA methodology to knock down SHC allows the conclusion that SHC is needed for ERα to localize in the plasma membrane.	topic_bc
78095	6	356085	6	NULL	NULL	0	NULL	statement 5	process		leads to					ER1	GP	upregulation of 			NULL		0	NULL	NULL	NULL	NULL	NULL	Deprivation of estrogen causes breast tumors in women to adapt and develop enhanced sensitivity to this steroid. Accordingly, women relapsing after treatment with oophorectomy, which substantially lowers estradiol for a prolonged period, respond secondarily to aromatase inhibitors with tumor regression. We have utilized in vitro and in vivo model systems to examine the biologic processes whereby Long Term Estradiol Deprivation (LTED) causes cells to adapts and develop hypersensitivity to estradiol. Several mechanisms are associated with this response including up-regulation of ERα and the MAP kinase, PI-3-kinase and mTOR growth factor pathways. ERα is 4–10 fold up-regulated as a result of demethylation of its C promoter, This nuclear receptor then co-opts a classical growth factor pathway using SHC, Grb-2 and Sos. This induces rapid nongenomic effects which are enhanced in LTED cells. The molecules involved in the nongenomic signaling process have been identified. Estradiol binds to cell membrance-associated ERα which physically associates with the adaptor protein SHC and induces its phosphorylation. In turn, SHC binds Grb-2 and Sos which results in the rapid activation of MAP kinase. These nongenomic effects of estradiol produce biologic effects as evidenced by Elk-1 activation and by morphologic changes in cell membrances. Additional effects include activation of the PI-3-kinase and mTOR pathways through estradiol-induced binding of ERα to the IGF-1 and EGF receptors. A major question is how ERα locates in the plasma membrance since it does not contain an inherent membrance localization signal. We have provided evidence that the IGF-1 receptor serves as an anchor for ERα in the plasma membrane. Estradiol causes phosphorylation of the adaptor protein, SHC and the IGF-1 receptor itself. SHC, after binding to ERα, serves as the “glue” which tethers ERα to SHC binding sites on the activated IFG-1 receptors. Use of siRNA methodology to knock down SHC allows the conclusion that SHC is needed for ERα to localize in the plasma membrane.	topic_bc
78096	7	356085	6	NULL	NULL	0	NULL	statement 5	process		leads to					MAP kinase	GP	upregulation of 			NULL		0	NULL	NULL	NULL	NULL	NULL	Deprivation of estrogen causes breast tumors in women to adapt and develop enhanced sensitivity to this steroid. Accordingly, women relapsing after treatment with oophorectomy, which substantially lowers estradiol for a prolonged period, respond secondarily to aromatase inhibitors with tumor regression. We have utilized in vitro and in vivo model systems to examine the biologic processes whereby Long Term Estradiol Deprivation (LTED) causes cells to adapts and develop hypersensitivity to estradiol. Several mechanisms are associated with this response including up-regulation of ERα and the MAP kinase, PI-3-kinase and mTOR growth factor pathways. ERα is 4–10 fold up-regulated as a result of demethylation of its C promoter, This nuclear receptor then co-opts a classical growth factor pathway using SHC, Grb-2 and Sos. This induces rapid nongenomic effects which are enhanced in LTED cells. The molecules involved in the nongenomic signaling process have been identified. Estradiol binds to cell membrance-associated ERα which physically associates with the adaptor protein SHC and induces its phosphorylation. In turn, SHC binds Grb-2 and Sos which results in the rapid activation of MAP kinase. These nongenomic effects of estradiol produce biologic effects as evidenced by Elk-1 activation and by morphologic changes in cell membrances. Additional effects include activation of the PI-3-kinase and mTOR pathways through estradiol-induced binding of ERα to the IGF-1 and EGF receptors. A major question is how ERα locates in the plasma membrance since it does not contain an inherent membrance localization signal. We have provided evidence that the IGF-1 receptor serves as an anchor for ERα in the plasma membrane. Estradiol causes phosphorylation of the adaptor protein, SHC and the IGF-1 receptor itself. SHC, after binding to ERα, serves as the “glue” which tethers ERα to SHC binding sites on the activated IFG-1 receptors. Use of siRNA methodology to knock down SHC allows the conclusion that SHC is needed for ERα to localize in the plasma membrane.	topic_bc
78097	8	356085	6	NULL	NULL	0	NULL	statement 5	process		leads to					PI-3 kinase pathway	process	upregulation of 			NULL		0	NULL	NULL	NULL	NULL	NULL	Deprivation of estrogen causes breast tumors in women to adapt and develop enhanced sensitivity to this steroid. Accordingly, women relapsing after treatment with oophorectomy, which substantially lowers estradiol for a prolonged period, respond secondarily to aromatase inhibitors with tumor regression. We have utilized in vitro and in vivo model systems to examine the biologic processes whereby Long Term Estradiol Deprivation (LTED) causes cells to adapts and develop hypersensitivity to estradiol. Several mechanisms are associated with this response including up-regulation of ERα and the MAP kinase, PI-3-kinase and mTOR growth factor pathways. ERα is 4–10 fold up-regulated as a result of demethylation of its C promoter, This nuclear receptor then co-opts a classical growth factor pathway using SHC, Grb-2 and Sos. This induces rapid nongenomic effects which are enhanced in LTED cells. The molecules involved in the nongenomic signaling process have been identified. Estradiol binds to cell membrance-associated ERα which physically associates with the adaptor protein SHC and induces its phosphorylation. In turn, SHC binds Grb-2 and Sos which results in the rapid activation of MAP kinase. These nongenomic effects of estradiol produce biologic effects as evidenced by Elk-1 activation and by morphologic changes in cell membrances. Additional effects include activation of the PI-3-kinase and mTOR pathways through estradiol-induced binding of ERα to the IGF-1 and EGF receptors. A major question is how ERα locates in the plasma membrance since it does not contain an inherent membrance localization signal. We have provided evidence that the IGF-1 receptor serves as an anchor for ERα in the plasma membrane. Estradiol causes phosphorylation of the adaptor protein, SHC and the IGF-1 receptor itself. SHC, after binding to ERα, serves as the “glue” which tethers ERα to SHC binding sites on the activated IFG-1 receptors. Use of siRNA methodology to knock down SHC allows the conclusion that SHC is needed for ERα to localize in the plasma membrane.	topic_bc
78098	9	356085	6	NULL	NULL	0	NULL	C promoter	GP	demethylation of	leads to					ER1	GP	upregulation of 			NULL		0	NULL	NULL	NULL	NULL	NULL	Deprivation of estrogen causes breast tumors in women to adapt and develop enhanced sensitivity to this steroid. Accordingly, women relapsing after treatment with oophorectomy, which substantially lowers estradiol for a prolonged period, respond secondarily to aromatase inhibitors with tumor regression. We have utilized in vitro and in vivo model systems to examine the biologic processes whereby Long Term Estradiol Deprivation (LTED) causes cells to adapts and develop hypersensitivity to estradiol. Several mechanisms are associated with this response including up-regulation of ERα and the MAP kinase, PI-3-kinase and mTOR growth factor pathways. ERα is 4–10 fold up-regulated as a result of demethylation of its C promoter, This nuclear receptor then co-opts a classical growth factor pathway using SHC, Grb-2 and Sos. This induces rapid nongenomic effects which are enhanced in LTED cells. The molecules involved in the nongenomic signaling process have been identified. Estradiol binds to cell membrance-associated ERα which physically associates with the adaptor protein SHC and induces its phosphorylation. In turn, SHC binds Grb-2 and Sos which results in the rapid activation of MAP kinase. These nongenomic effects of estradiol produce biologic effects as evidenced by Elk-1 activation and by morphologic changes in cell membrances. Additional effects include activation of the PI-3-kinase and mTOR pathways through estradiol-induced binding of ERα to the IGF-1 and EGF receptors. A major question is how ERα locates in the plasma membrance since it does not contain an inherent membrance localization signal. We have provided evidence that the IGF-1 receptor serves as an anchor for ERα in the plasma membrane. Estradiol causes phosphorylation of the adaptor protein, SHC and the IGF-1 receptor itself. SHC, after binding to ERα, serves as the “glue” which tethers ERα to SHC binding sites on the activated IFG-1 receptors. Use of siRNA methodology to knock down SHC allows the conclusion that SHC is needed for ERα to localize in the plasma membrane.	topic_bc
78099	10	356085	6	NULL	NULL	0	NULL	SHC	GP		bind					Grb-2	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Deprivation of estrogen causes breast tumors in women to adapt and develop enhanced sensitivity to this steroid. Accordingly, women relapsing after treatment with oophorectomy, which substantially lowers estradiol for a prolonged period, respond secondarily to aromatase inhibitors with tumor regression. We have utilized in vitro and in vivo model systems to examine the biologic processes whereby Long Term Estradiol Deprivation (LTED) causes cells to adapts and develop hypersensitivity to estradiol. Several mechanisms are associated with this response including up-regulation of ERα and the MAP kinase, PI-3-kinase and mTOR growth factor pathways. ERα is 4–10 fold up-regulated as a result of demethylation of its C promoter, This nuclear receptor then co-opts a classical growth factor pathway using SHC, Grb-2 and Sos. This induces rapid nongenomic effects which are enhanced in LTED cells. The molecules involved in the nongenomic signaling process have been identified. Estradiol binds to cell membrance-associated ERα which physically associates with the adaptor protein SHC and induces its phosphorylation. In turn, SHC binds Grb-2 and Sos which results in the rapid activation of MAP kinase. These nongenomic effects of estradiol produce biologic effects as evidenced by Elk-1 activation and by morphologic changes in cell membrances. Additional effects include activation of the PI-3-kinase and mTOR pathways through estradiol-induced binding of ERα to the IGF-1 and EGF receptors. A major question is how ERα locates in the plasma membrance since it does not contain an inherent membrance localization signal. We have provided evidence that the IGF-1 receptor serves as an anchor for ERα in the plasma membrane. Estradiol causes phosphorylation of the adaptor protein, SHC and the IGF-1 receptor itself. SHC, after binding to ERα, serves as the “glue” which tethers ERα to SHC binding sites on the activated IFG-1 receptors. Use of siRNA methodology to knock down SHC allows the conclusion that SHC is needed for ERα to localize in the plasma membrane.	topic_bc
78100	11	356085	6	NULL	NULL	0	NULL	SHC	GP		bind					Sos	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Deprivation of estrogen causes breast tumors in women to adapt and develop enhanced sensitivity to this steroid. Accordingly, women relapsing after treatment with oophorectomy, which substantially lowers estradiol for a prolonged period, respond secondarily to aromatase inhibitors with tumor regression. We have utilized in vitro and in vivo model systems to examine the biologic processes whereby Long Term Estradiol Deprivation (LTED) causes cells to adapts and develop hypersensitivity to estradiol. Several mechanisms are associated with this response including up-regulation of ERα and the MAP kinase, PI-3-kinase and mTOR growth factor pathways. ERα is 4–10 fold up-regulated as a result of demethylation of its C promoter, This nuclear receptor then co-opts a classical growth factor pathway using SHC, Grb-2 and Sos. This induces rapid nongenomic effects which are enhanced in LTED cells. The molecules involved in the nongenomic signaling process have been identified. Estradiol binds to cell membrance-associated ERα which physically associates with the adaptor protein SHC and induces its phosphorylation. In turn, SHC binds Grb-2 and Sos which results in the rapid activation of MAP kinase. These nongenomic effects of estradiol produce biologic effects as evidenced by Elk-1 activation and by morphologic changes in cell membrances. Additional effects include activation of the PI-3-kinase and mTOR pathways through estradiol-induced binding of ERα to the IGF-1 and EGF receptors. A major question is how ERα locates in the plasma membrance since it does not contain an inherent membrance localization signal. We have provided evidence that the IGF-1 receptor serves as an anchor for ERα in the plasma membrane. Estradiol causes phosphorylation of the adaptor protein, SHC and the IGF-1 receptor itself. SHC, after binding to ERα, serves as the “glue” which tethers ERα to SHC binding sites on the activated IFG-1 receptors. Use of siRNA methodology to knock down SHC allows the conclusion that SHC is needed for ERα to localize in the plasma membrane.	topic_bc
78101	12	356085	6	NULL	NULL	0	NULL	statement 10	process		leads to					MAP kinase	GP	activation of 			NULL		0	NULL	NULL	NULL	NULL	NULL	Deprivation of estrogen causes breast tumors in women to adapt and develop enhanced sensitivity to this steroid. Accordingly, women relapsing after treatment with oophorectomy, which substantially lowers estradiol for a prolonged period, respond secondarily to aromatase inhibitors with tumor regression. We have utilized in vitro and in vivo model systems to examine the biologic processes whereby Long Term Estradiol Deprivation (LTED) causes cells to adapts and develop hypersensitivity to estradiol. Several mechanisms are associated with this response including up-regulation of ERα and the MAP kinase, PI-3-kinase and mTOR growth factor pathways. ERα is 4–10 fold up-regulated as a result of demethylation of its C promoter, This nuclear receptor then co-opts a classical growth factor pathway using SHC, Grb-2 and Sos. This induces rapid nongenomic effects which are enhanced in LTED cells. The molecules involved in the nongenomic signaling process have been identified. Estradiol binds to cell membrance-associated ERα which physically associates with the adaptor protein SHC and induces its phosphorylation. In turn, SHC binds Grb-2 and Sos which results in the rapid activation of MAP kinase. These nongenomic effects of estradiol produce biologic effects as evidenced by Elk-1 activation and by morphologic changes in cell membrances. Additional effects include activation of the PI-3-kinase and mTOR pathways through estradiol-induced binding of ERα to the IGF-1 and EGF receptors. A major question is how ERα locates in the plasma membrance since it does not contain an inherent membrance localization signal. We have provided evidence that the IGF-1 receptor serves as an anchor for ERα in the plasma membrane. Estradiol causes phosphorylation of the adaptor protein, SHC and the IGF-1 receptor itself. SHC, after binding to ERα, serves as the “glue” which tethers ERα to SHC binding sites on the activated IFG-1 receptors. Use of siRNA methodology to knock down SHC allows the conclusion that SHC is needed for ERα to localize in the plasma membrane.	topic_bc
78102	13	356085	6	NULL	NULL	0	NULL	ER1	GP		bind					IGF-1	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Deprivation of estrogen causes breast tumors in women to adapt and develop enhanced sensitivity to this steroid. Accordingly, women relapsing after treatment with oophorectomy, which substantially lowers estradiol for a prolonged period, respond secondarily to aromatase inhibitors with tumor regression. We have utilized in vitro and in vivo model systems to examine the biologic processes whereby Long Term Estradiol Deprivation (LTED) causes cells to adapts and develop hypersensitivity to estradiol. Several mechanisms are associated with this response including up-regulation of ERα and the MAP kinase, PI-3-kinase and mTOR growth factor pathways. ERα is 4–10 fold up-regulated as a result of demethylation of its C promoter, This nuclear receptor then co-opts a classical growth factor pathway using SHC, Grb-2 and Sos. This induces rapid nongenomic effects which are enhanced in LTED cells. The molecules involved in the nongenomic signaling process have been identified. Estradiol binds to cell membrance-associated ERα which physically associates with the adaptor protein SHC and induces its phosphorylation. In turn, SHC binds Grb-2 and Sos which results in the rapid activation of MAP kinase. These nongenomic effects of estradiol produce biologic effects as evidenced by Elk-1 activation and by morphologic changes in cell membrances. Additional effects include activation of the PI-3-kinase and mTOR pathways through estradiol-induced binding of ERα to the IGF-1 and EGF receptors. A major question is how ERα locates in the plasma membrance since it does not contain an inherent membrance localization signal. We have provided evidence that the IGF-1 receptor serves as an anchor for ERα in the plasma membrane. Estradiol causes phosphorylation of the adaptor protein, SHC and the IGF-1 receptor itself. SHC, after binding to ERα, serves as the “glue” which tethers ERα to SHC binding sites on the activated IFG-1 receptors. Use of siRNA methodology to knock down SHC allows the conclusion that SHC is needed for ERα to localize in the plasma membrane.	topic_bc
78103	14	356085	6	NULL	NULL	0	NULL	ER1	GP		bind					EGF receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Deprivation of estrogen causes breast tumors in women to adapt and develop enhanced sensitivity to this steroid. Accordingly, women relapsing after treatment with oophorectomy, which substantially lowers estradiol for a prolonged period, respond secondarily to aromatase inhibitors with tumor regression. We have utilized in vitro and in vivo model systems to examine the biologic processes whereby Long Term Estradiol Deprivation (LTED) causes cells to adapts and develop hypersensitivity to estradiol. Several mechanisms are associated with this response including up-regulation of ERα and the MAP kinase, PI-3-kinase and mTOR growth factor pathways. ERα is 4–10 fold up-regulated as a result of demethylation of its C promoter, This nuclear receptor then co-opts a classical growth factor pathway using SHC, Grb-2 and Sos. This induces rapid nongenomic effects which are enhanced in LTED cells. The molecules involved in the nongenomic signaling process have been identified. Estradiol binds to cell membrance-associated ERα which physically associates with the adaptor protein SHC and induces its phosphorylation. In turn, SHC binds Grb-2 and Sos which results in the rapid activation of MAP kinase. These nongenomic effects of estradiol produce biologic effects as evidenced by Elk-1 activation and by morphologic changes in cell membrances. Additional effects include activation of the PI-3-kinase and mTOR pathways through estradiol-induced binding of ERα to the IGF-1 and EGF receptors. A major question is how ERα locates in the plasma membrance since it does not contain an inherent membrance localization signal. We have provided evidence that the IGF-1 receptor serves as an anchor for ERα in the plasma membrane. Estradiol causes phosphorylation of the adaptor protein, SHC and the IGF-1 receptor itself. SHC, after binding to ERα, serves as the “glue” which tethers ERα to SHC binding sites on the activated IFG-1 receptors. Use of siRNA methodology to knock down SHC allows the conclusion that SHC is needed for ERα to localize in the plasma membrane.	topic_bc
78104	15	356085	6	NULL	NULL	0	NULL	statement 13	process		is induced by					estradiol	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Deprivation of estrogen causes breast tumors in women to adapt and develop enhanced sensitivity to this steroid. Accordingly, women relapsing after treatment with oophorectomy, which substantially lowers estradiol for a prolonged period, respond secondarily to aromatase inhibitors with tumor regression. We have utilized in vitro and in vivo model systems to examine the biologic processes whereby Long Term Estradiol Deprivation (LTED) causes cells to adapts and develop hypersensitivity to estradiol. Several mechanisms are associated with this response including up-regulation of ERα and the MAP kinase, PI-3-kinase and mTOR growth factor pathways. ERα is 4–10 fold up-regulated as a result of demethylation of its C promoter, This nuclear receptor then co-opts a classical growth factor pathway using SHC, Grb-2 and Sos. This induces rapid nongenomic effects which are enhanced in LTED cells. The molecules involved in the nongenomic signaling process have been identified. Estradiol binds to cell membrance-associated ERα which physically associates with the adaptor protein SHC and induces its phosphorylation. In turn, SHC binds Grb-2 and Sos which results in the rapid activation of MAP kinase. These nongenomic effects of estradiol produce biologic effects as evidenced by Elk-1 activation and by morphologic changes in cell membrances. Additional effects include activation of the PI-3-kinase and mTOR pathways through estradiol-induced binding of ERα to the IGF-1 and EGF receptors. A major question is how ERα locates in the plasma membrance since it does not contain an inherent membrance localization signal. We have provided evidence that the IGF-1 receptor serves as an anchor for ERα in the plasma membrane. Estradiol causes phosphorylation of the adaptor protein, SHC and the IGF-1 receptor itself. SHC, after binding to ERα, serves as the “glue” which tethers ERα to SHC binding sites on the activated IFG-1 receptors. Use of siRNA methodology to knock down SHC allows the conclusion that SHC is needed for ERα to localize in the plasma membrane.	topic_bc
78105	16	356085	6	NULL	NULL	0	NULL	statement 14	process		is induced by					estradiol	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Deprivation of estrogen causes breast tumors in women to adapt and develop enhanced sensitivity to this steroid. Accordingly, women relapsing after treatment with oophorectomy, which substantially lowers estradiol for a prolonged period, respond secondarily to aromatase inhibitors with tumor regression. We have utilized in vitro and in vivo model systems to examine the biologic processes whereby Long Term Estradiol Deprivation (LTED) causes cells to adapts and develop hypersensitivity to estradiol. Several mechanisms are associated with this response including up-regulation of ERα and the MAP kinase, PI-3-kinase and mTOR growth factor pathways. ERα is 4–10 fold up-regulated as a result of demethylation of its C promoter, This nuclear receptor then co-opts a classical growth factor pathway using SHC, Grb-2 and Sos. This induces rapid nongenomic effects which are enhanced in LTED cells. The molecules involved in the nongenomic signaling process have been identified. Estradiol binds to cell membrance-associated ERα which physically associates with the adaptor protein SHC and induces its phosphorylation. In turn, SHC binds Grb-2 and Sos which results in the rapid activation of MAP kinase. These nongenomic effects of estradiol produce biologic effects as evidenced by Elk-1 activation and by morphologic changes in cell membrances. Additional effects include activation of the PI-3-kinase and mTOR pathways through estradiol-induced binding of ERα to the IGF-1 and EGF receptors. A major question is how ERα locates in the plasma membrance since it does not contain an inherent membrance localization signal. We have provided evidence that the IGF-1 receptor serves as an anchor for ERα in the plasma membrane. Estradiol causes phosphorylation of the adaptor protein, SHC and the IGF-1 receptor itself. SHC, after binding to ERα, serves as the “glue” which tethers ERα to SHC binding sites on the activated IFG-1 receptors. Use of siRNA methodology to knock down SHC allows the conclusion that SHC is needed for ERα to localize in the plasma membrane.	topic_bc
78106	17	356085	6	NULL	NULL	0	NULL	statement 13	process		activates					PI-3-kinase	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Deprivation of estrogen causes breast tumors in women to adapt and develop enhanced sensitivity to this steroid. Accordingly, women relapsing after treatment with oophorectomy, which substantially lowers estradiol for a prolonged period, respond secondarily to aromatase inhibitors with tumor regression. We have utilized in vitro and in vivo model systems to examine the biologic processes whereby Long Term Estradiol Deprivation (LTED) causes cells to adapts and develop hypersensitivity to estradiol. Several mechanisms are associated with this response including up-regulation of ERα and the MAP kinase, PI-3-kinase and mTOR growth factor pathways. ERα is 4–10 fold up-regulated as a result of demethylation of its C promoter, This nuclear receptor then co-opts a classical growth factor pathway using SHC, Grb-2 and Sos. This induces rapid nongenomic effects which are enhanced in LTED cells. The molecules involved in the nongenomic signaling process have been identified. Estradiol binds to cell membrance-associated ERα which physically associates with the adaptor protein SHC and induces its phosphorylation. In turn, SHC binds Grb-2 and Sos which results in the rapid activation of MAP kinase. These nongenomic effects of estradiol produce biologic effects as evidenced by Elk-1 activation and by morphologic changes in cell membrances. Additional effects include activation of the PI-3-kinase and mTOR pathways through estradiol-induced binding of ERα to the IGF-1 and EGF receptors. A major question is how ERα locates in the plasma membrance since it does not contain an inherent membrance localization signal. We have provided evidence that the IGF-1 receptor serves as an anchor for ERα in the plasma membrane. Estradiol causes phosphorylation of the adaptor protein, SHC and the IGF-1 receptor itself. SHC, after binding to ERα, serves as the “glue” which tethers ERα to SHC binding sites on the activated IFG-1 receptors. Use of siRNA methodology to knock down SHC allows the conclusion that SHC is needed for ERα to localize in the plasma membrane.	topic_bc
78107	18	356085	6	NULL	NULL	0	NULL	statement 13	process		activates					mTOR pathway	process				NULL		0	NULL	NULL	NULL	NULL	NULL	Deprivation of estrogen causes breast tumors in women to adapt and develop enhanced sensitivity to this steroid. Accordingly, women relapsing after treatment with oophorectomy, which substantially lowers estradiol for a prolonged period, respond secondarily to aromatase inhibitors with tumor regression. We have utilized in vitro and in vivo model systems to examine the biologic processes whereby Long Term Estradiol Deprivation (LTED) causes cells to adapts and develop hypersensitivity to estradiol. Several mechanisms are associated with this response including up-regulation of ERα and the MAP kinase, PI-3-kinase and mTOR growth factor pathways. ERα is 4–10 fold up-regulated as a result of demethylation of its C promoter, This nuclear receptor then co-opts a classical growth factor pathway using SHC, Grb-2 and Sos. This induces rapid nongenomic effects which are enhanced in LTED cells. The molecules involved in the nongenomic signaling process have been identified. Estradiol binds to cell membrance-associated ERα which physically associates with the adaptor protein SHC and induces its phosphorylation. In turn, SHC binds Grb-2 and Sos which results in the rapid activation of MAP kinase. These nongenomic effects of estradiol produce biologic effects as evidenced by Elk-1 activation and by morphologic changes in cell membrances. Additional effects include activation of the PI-3-kinase and mTOR pathways through estradiol-induced binding of ERα to the IGF-1 and EGF receptors. A major question is how ERα locates in the plasma membrance since it does not contain an inherent membrance localization signal. We have provided evidence that the IGF-1 receptor serves as an anchor for ERα in the plasma membrane. Estradiol causes phosphorylation of the adaptor protein, SHC and the IGF-1 receptor itself. SHC, after binding to ERα, serves as the “glue” which tethers ERα to SHC binding sites on the activated IFG-1 receptors. Use of siRNA methodology to knock down SHC allows the conclusion that SHC is needed for ERα to localize in the plasma membrane.	topic_bc
78108	19	356085	6	NULL	NULL	0	NULL	statement 14	process		activates					PI-3 kinase pathway	process				NULL		0	NULL	NULL	NULL	NULL	NULL	Deprivation of estrogen causes breast tumors in women to adapt and develop enhanced sensitivity to this steroid. Accordingly, women relapsing after treatment with oophorectomy, which substantially lowers estradiol for a prolonged period, respond secondarily to aromatase inhibitors with tumor regression. We have utilized in vitro and in vivo model systems to examine the biologic processes whereby Long Term Estradiol Deprivation (LTED) causes cells to adapts and develop hypersensitivity to estradiol. Several mechanisms are associated with this response including up-regulation of ERα and the MAP kinase, PI-3-kinase and mTOR growth factor pathways. ERα is 4–10 fold up-regulated as a result of demethylation of its C promoter, This nuclear receptor then co-opts a classical growth factor pathway using SHC, Grb-2 and Sos. This induces rapid nongenomic effects which are enhanced in LTED cells. The molecules involved in the nongenomic signaling process have been identified. Estradiol binds to cell membrance-associated ERα which physically associates with the adaptor protein SHC and induces its phosphorylation. In turn, SHC binds Grb-2 and Sos which results in the rapid activation of MAP kinase. These nongenomic effects of estradiol produce biologic effects as evidenced by Elk-1 activation and by morphologic changes in cell membrances. Additional effects include activation of the PI-3-kinase and mTOR pathways through estradiol-induced binding of ERα to the IGF-1 and EGF receptors. A major question is how ERα locates in the plasma membrance since it does not contain an inherent membrance localization signal. We have provided evidence that the IGF-1 receptor serves as an anchor for ERα in the plasma membrane. Estradiol causes phosphorylation of the adaptor protein, SHC and the IGF-1 receptor itself. SHC, after binding to ERα, serves as the “glue” which tethers ERα to SHC binding sites on the activated IFG-1 receptors. Use of siRNA methodology to knock down SHC allows the conclusion that SHC is needed for ERα to localize in the plasma membrane.	topic_bc
78109	20	356085	6	NULL	NULL	0	NULL	statement 14	process		activates					mTOR pathway	process				NULL		0	NULL	NULL	NULL	NULL	NULL	Deprivation of estrogen causes breast tumors in women to adapt and develop enhanced sensitivity to this steroid. Accordingly, women relapsing after treatment with oophorectomy, which substantially lowers estradiol for a prolonged period, respond secondarily to aromatase inhibitors with tumor regression. We have utilized in vitro and in vivo model systems to examine the biologic processes whereby Long Term Estradiol Deprivation (LTED) causes cells to adapts and develop hypersensitivity to estradiol. Several mechanisms are associated with this response including up-regulation of ERα and the MAP kinase, PI-3-kinase and mTOR growth factor pathways. ERα is 4–10 fold up-regulated as a result of demethylation of its C promoter, This nuclear receptor then co-opts a classical growth factor pathway using SHC, Grb-2 and Sos. This induces rapid nongenomic effects which are enhanced in LTED cells. The molecules involved in the nongenomic signaling process have been identified. Estradiol binds to cell membrance-associated ERα which physically associates with the adaptor protein SHC and induces its phosphorylation. In turn, SHC binds Grb-2 and Sos which results in the rapid activation of MAP kinase. These nongenomic effects of estradiol produce biologic effects as evidenced by Elk-1 activation and by morphologic changes in cell membrances. Additional effects include activation of the PI-3-kinase and mTOR pathways through estradiol-induced binding of ERα to the IGF-1 and EGF receptors. A major question is how ERα locates in the plasma membrance since it does not contain an inherent membrance localization signal. We have provided evidence that the IGF-1 receptor serves as an anchor for ERα in the plasma membrane. Estradiol causes phosphorylation of the adaptor protein, SHC and the IGF-1 receptor itself. SHC, after binding to ERα, serves as the “glue” which tethers ERα to SHC binding sites on the activated IFG-1 receptors. Use of siRNA methodology to knock down SHC allows the conclusion that SHC is needed for ERα to localize in the plasma membrane.	topic_bc
78110	21	356085	6	NULL	NULL	0	NULL	ER1	GP		is localized to					plasma membrane	CellComponent				NULL		0	NULL	NULL	NULL	NULL	NULL	Deprivation of estrogen causes breast tumors in women to adapt and develop enhanced sensitivity to this steroid. Accordingly, women relapsing after treatment with oophorectomy, which substantially lowers estradiol for a prolonged period, respond secondarily to aromatase inhibitors with tumor regression. We have utilized in vitro and in vivo model systems to examine the biologic processes whereby Long Term Estradiol Deprivation (LTED) causes cells to adapts and develop hypersensitivity to estradiol. Several mechanisms are associated with this response including up-regulation of ERα and the MAP kinase, PI-3-kinase and mTOR growth factor pathways. ERα is 4–10 fold up-regulated as a result of demethylation of its C promoter, This nuclear receptor then co-opts a classical growth factor pathway using SHC, Grb-2 and Sos. This induces rapid nongenomic effects which are enhanced in LTED cells. The molecules involved in the nongenomic signaling process have been identified. Estradiol binds to cell membrance-associated ERα which physically associates with the adaptor protein SHC and induces its phosphorylation. In turn, SHC binds Grb-2 and Sos which results in the rapid activation of MAP kinase. These nongenomic effects of estradiol produce biologic effects as evidenced by Elk-1 activation and by morphologic changes in cell membrances. Additional effects include activation of the PI-3-kinase and mTOR pathways through estradiol-induced binding of ERα to the IGF-1 and EGF receptors. A major question is how ERα locates in the plasma membrance since it does not contain an inherent membrance localization signal. We have provided evidence that the IGF-1 receptor serves as an anchor for ERα in the plasma membrane. Estradiol causes phosphorylation of the adaptor protein, SHC and the IGF-1 receptor itself. SHC, after binding to ERα, serves as the “glue” which tethers ERα to SHC binding sites on the activated IFG-1 receptors. Use of siRNA methodology to knock down SHC allows the conclusion that SHC is needed for ERα to localize in the plasma membrane.	topic_bc
78111	22	356085	6	NULL	NULL	0	NULL	estradiol	Chemical		causes					SHC	GP	phosphorylation of			NULL		0	NULL	NULL	NULL	NULL	NULL	Deprivation of estrogen causes breast tumors in women to adapt and develop enhanced sensitivity to this steroid. Accordingly, women relapsing after treatment with oophorectomy, which substantially lowers estradiol for a prolonged period, respond secondarily to aromatase inhibitors with tumor regression. We have utilized in vitro and in vivo model systems to examine the biologic processes whereby Long Term Estradiol Deprivation (LTED) causes cells to adapts and develop hypersensitivity to estradiol. Several mechanisms are associated with this response including up-regulation of ERα and the MAP kinase, PI-3-kinase and mTOR growth factor pathways. ERα is 4–10 fold up-regulated as a result of demethylation of its C promoter, This nuclear receptor then co-opts a classical growth factor pathway using SHC, Grb-2 and Sos. This induces rapid nongenomic effects which are enhanced in LTED cells. The molecules involved in the nongenomic signaling process have been identified. Estradiol binds to cell membrance-associated ERα which physically associates with the adaptor protein SHC and induces its phosphorylation. In turn, SHC binds Grb-2 and Sos which results in the rapid activation of MAP kinase. These nongenomic effects of estradiol produce biologic effects as evidenced by Elk-1 activation and by morphologic changes in cell membrances. Additional effects include activation of the PI-3-kinase and mTOR pathways through estradiol-induced binding of ERα to the IGF-1 and EGF receptors. A major question is how ERα locates in the plasma membrance since it does not contain an inherent membrance localization signal. We have provided evidence that the IGF-1 receptor serves as an anchor for ERα in the plasma membrane. Estradiol causes phosphorylation of the adaptor protein, SHC and the IGF-1 receptor itself. SHC, after binding to ERα, serves as the “glue” which tethers ERα to SHC binding sites on the activated IFG-1 receptors. Use of siRNA methodology to knock down SHC allows the conclusion that SHC is needed for ERα to localize in the plasma membrane.	topic_bc
78112	23	356085	6	NULL	NULL	0	NULL	estradiol	Chemical		causes					IGF-1	GP	phosphorylation of			NULL		0	NULL	NULL	NULL	NULL	NULL	Deprivation of estrogen causes breast tumors in women to adapt and develop enhanced sensitivity to this steroid. Accordingly, women relapsing after treatment with oophorectomy, which substantially lowers estradiol for a prolonged period, respond secondarily to aromatase inhibitors with tumor regression. We have utilized in vitro and in vivo model systems to examine the biologic processes whereby Long Term Estradiol Deprivation (LTED) causes cells to adapts and develop hypersensitivity to estradiol. Several mechanisms are associated with this response including up-regulation of ERα and the MAP kinase, PI-3-kinase and mTOR growth factor pathways. ERα is 4–10 fold up-regulated as a result of demethylation of its C promoter, This nuclear receptor then co-opts a classical growth factor pathway using SHC, Grb-2 and Sos. This induces rapid nongenomic effects which are enhanced in LTED cells. The molecules involved in the nongenomic signaling process have been identified. Estradiol binds to cell membrance-associated ERα which physically associates with the adaptor protein SHC and induces its phosphorylation. In turn, SHC binds Grb-2 and Sos which results in the rapid activation of MAP kinase. These nongenomic effects of estradiol produce biologic effects as evidenced by Elk-1 activation and by morphologic changes in cell membrances. Additional effects include activation of the PI-3-kinase and mTOR pathways through estradiol-induced binding of ERα to the IGF-1 and EGF receptors. A major question is how ERα locates in the plasma membrance since it does not contain an inherent membrance localization signal. We have provided evidence that the IGF-1 receptor serves as an anchor for ERα in the plasma membrane. Estradiol causes phosphorylation of the adaptor protein, SHC and the IGF-1 receptor itself. SHC, after binding to ERα, serves as the “glue” which tethers ERα to SHC binding sites on the activated IFG-1 receptors. Use of siRNA methodology to knock down SHC allows the conclusion that SHC is needed for ERα to localize in the plasma membrane.	topic_bc
78113	24	356085	6	NULL	NULL	0	NULL	SHC	GP		is a type of					adaptor protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Deprivation of estrogen causes breast tumors in women to adapt and develop enhanced sensitivity to this steroid. Accordingly, women relapsing after treatment with oophorectomy, which substantially lowers estradiol for a prolonged period, respond secondarily to aromatase inhibitors with tumor regression. We have utilized in vitro and in vivo model systems to examine the biologic processes whereby Long Term Estradiol Deprivation (LTED) causes cells to adapts and develop hypersensitivity to estradiol. Several mechanisms are associated with this response including up-regulation of ERα and the MAP kinase, PI-3-kinase and mTOR growth factor pathways. ERα is 4–10 fold up-regulated as a result of demethylation of its C promoter, This nuclear receptor then co-opts a classical growth factor pathway using SHC, Grb-2 and Sos. This induces rapid nongenomic effects which are enhanced in LTED cells. The molecules involved in the nongenomic signaling process have been identified. Estradiol binds to cell membrance-associated ERα which physically associates with the adaptor protein SHC and induces its phosphorylation. In turn, SHC binds Grb-2 and Sos which results in the rapid activation of MAP kinase. These nongenomic effects of estradiol produce biologic effects as evidenced by Elk-1 activation and by morphologic changes in cell membrances. Additional effects include activation of the PI-3-kinase and mTOR pathways through estradiol-induced binding of ERα to the IGF-1 and EGF receptors. A major question is how ERα locates in the plasma membrance since it does not contain an inherent membrance localization signal. We have provided evidence that the IGF-1 receptor serves as an anchor for ERα in the plasma membrane. Estradiol causes phosphorylation of the adaptor protein, SHC and the IGF-1 receptor itself. SHC, after binding to ERα, serves as the “glue” which tethers ERα to SHC binding sites on the activated IFG-1 receptors. Use of siRNA methodology to knock down SHC allows the conclusion that SHC is needed for ERα to localize in the plasma membrane.	topic_bc
78114	25	356085	6	NULL	NULL	0	NULL	IGF-1	GP		is a type of					adaptor protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Deprivation of estrogen causes breast tumors in women to adapt and develop enhanced sensitivity to this steroid. Accordingly, women relapsing after treatment with oophorectomy, which substantially lowers estradiol for a prolonged period, respond secondarily to aromatase inhibitors with tumor regression. We have utilized in vitro and in vivo model systems to examine the biologic processes whereby Long Term Estradiol Deprivation (LTED) causes cells to adapts and develop hypersensitivity to estradiol. Several mechanisms are associated with this response including up-regulation of ERα and the MAP kinase, PI-3-kinase and mTOR growth factor pathways. ERα is 4–10 fold up-regulated as a result of demethylation of its C promoter, This nuclear receptor then co-opts a classical growth factor pathway using SHC, Grb-2 and Sos. This induces rapid nongenomic effects which are enhanced in LTED cells. The molecules involved in the nongenomic signaling process have been identified. Estradiol binds to cell membrance-associated ERα which physically associates with the adaptor protein SHC and induces its phosphorylation. In turn, SHC binds Grb-2 and Sos which results in the rapid activation of MAP kinase. These nongenomic effects of estradiol produce biologic effects as evidenced by Elk-1 activation and by morphologic changes in cell membrances. Additional effects include activation of the PI-3-kinase and mTOR pathways through estradiol-induced binding of ERα to the IGF-1 and EGF receptors. A major question is how ERα locates in the plasma membrance since it does not contain an inherent membrance localization signal. We have provided evidence that the IGF-1 receptor serves as an anchor for ERα in the plasma membrane. Estradiol causes phosphorylation of the adaptor protein, SHC and the IGF-1 receptor itself. SHC, after binding to ERα, serves as the “glue” which tethers ERα to SHC binding sites on the activated IFG-1 receptors. Use of siRNA methodology to knock down SHC allows the conclusion that SHC is needed for ERα to localize in the plasma membrane.	topic_bc
78086	1	356086	6	NULL	NULL	0	NULL	 rs13387042			is located on					chromosome 2q35	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	Familial clustering studies indicate that breast cancer risk has a substantial genetic component1, 2, 3. To identify new breast cancer risk variants, we genotyped approximately 300,000 SNPs in 1,600 Icelandic individuals with breast cancer and 11,563 controls using the Illumina Hap300 platform. We then tested selected SNPs in five replication sample sets. Overall, we studied 4,554 affected individuals and 17,577 controls. Two SNPs consistently associated with breast cancer: 25% of individuals of European descent are homozygous for allele A of rs13387042 on chromosome 2q35 and have an estimated 1.44-fold greater risk than noncarriers, and for allele T of rs3803662 on 16q12, about 7% are homozygous and have a 1.64-fold greater risk. Risk from both alleles was confined to estrogen receptor–positive tumors. At present, no genes have been identified in the linkage disequilibrium block containing rs13387042. rs3803662 is near the 5' end of TNRC9, a high mobility group chromatin–associated protein whose expression is implicated in breast cancer metastasis to bone4.	topic_bc
78087	2	356086	6	NULL	NULL	NULL	NULL	 rs3803662			is located on					Chromosome 16q12	Chromosome				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Familial clustering studies indicate that breast cancer risk has a substantial genetic component1, 2, 3. To identify new breast cancer risk variants, we genotyped approximately 300,000 SNPs in 1,600 Icelandic individuals with breast cancer and 11,563 controls using the Illumina Hap300 platform. We then tested selected SNPs in five replication sample sets. Overall, we studied 4,554 affected individuals and 17,577 controls. Two SNPs consistently associated with breast cancer: 25% of individuals of European descent are homozygous for allele A of rs13387042 on chromosome 2q35 and have an estimated 1.44-fold greater risk than noncarriers, and for allele T of rs3803662 on 16q12, about 7% are homozygous and have a 1.64-fold greater risk. Risk from both alleles was confined to estrogen receptor–positive tumors. At present, no genes have been identified in the linkage disequilibrium block containing rs13387042. rs3803662 is near the 5' end of TNRC9, a high mobility group chromatin–associated protein whose expression is implicated in breast cancer metastasis to bone4.	topic_bc
78088	3	356086	6	NULL	NULL	0	NULL	statement 1	process		leads to					 estrogen receptor positive tumor	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Familial clustering studies indicate that breast cancer risk has a substantial genetic component1, 2, 3. To identify new breast cancer risk variants, we genotyped approximately 300,000 SNPs in 1,600 Icelandic individuals with breast cancer and 11,563 controls using the Illumina Hap300 platform. We then tested selected SNPs in five replication sample sets. Overall, we studied 4,554 affected individuals and 17,577 controls. Two SNPs consistently associated with breast cancer: 25% of individuals of European descent are homozygous for allele A of rs13387042 on chromosome 2q35 and have an estimated 1.44-fold greater risk than noncarriers, and for allele T of rs3803662 on 16q12, about 7% are homozygous and have a 1.64-fold greater risk. Risk from both alleles was confined to estrogen receptor–positive tumors. At present, no genes have been identified in the linkage disequilibrium block containing rs13387042. rs3803662 is near the 5' end of TNRC9, a high mobility group chromatin–associated protein whose expression is implicated in breast cancer metastasis to bone4.	topic_bc
78089	4	356086	6	NULL	NULL	0	NULL	statement 2	process		leads to					 estrogen receptor positive tumor	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Familial clustering studies indicate that breast cancer risk has a substantial genetic component1, 2, 3. To identify new breast cancer risk variants, we genotyped approximately 300,000 SNPs in 1,600 Icelandic individuals with breast cancer and 11,563 controls using the Illumina Hap300 platform. We then tested selected SNPs in five replication sample sets. Overall, we studied 4,554 affected individuals and 17,577 controls. Two SNPs consistently associated with breast cancer: 25% of individuals of European descent are homozygous for allele A of rs13387042 on chromosome 2q35 and have an estimated 1.44-fold greater risk than noncarriers, and for allele T of rs3803662 on 16q12, about 7% are homozygous and have a 1.64-fold greater risk. Risk from both alleles was confined to estrogen receptor–positive tumors. At present, no genes have been identified in the linkage disequilibrium block containing rs13387042. rs3803662 is near the 5' end of TNRC9, a high mobility group chromatin–associated protein whose expression is implicated in breast cancer metastasis to bone4.	topic_bc
77064	1	356087	5	NULL	NULL	0	NULL	IL-6	GP	levels of;;serum	is increased in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Several reports described increased serum IL-6 levels in schizophrenia (Cazzullo et al., 1998). IL-6 serum levels might be especially high in patients with an unfavourable course of the disease (Lin et al., 1998) and in patients with a long duration of the disease (Ganguli et al., 1994).	topic_sch
77065	2	356087	5	NULL	NULL	0	NULL	IL-6	GP	levels of;;serum	is higher in					schizophrenia	MedicalFinding	patients of;;unfavourable course of			NULL		0	NULL	NULL	NULL	NULL	NULL	Several reports described increased serum IL-6 levels in schizophrenia (Cazzullo et al., 1998). IL-6 serum levels might be especially high in patients with an unfavourable course of the disease (Lin et al., 1998) and in patients with a long duration of the disease (Ganguli et al., 1994).	topic_sch
77066	3	356087	5	NULL	NULL	0	NULL	IL-6	GP	levels of;;serum	is higher in					schizophrenia	MedicalFinding	patients of;;long duration of			NULL		0	NULL	NULL	NULL	NULL	NULL	Several reports described increased serum IL-6 levels in schizophrenia (Cazzullo et al., 1998). IL-6 serum levels might be especially high in patients with an unfavourable course of the disease (Lin et al., 1998) and in patients with a long duration of the disease (Ganguli et al., 1994).	topic_sch
77067	1	356088	5	NULL	NULL	0	NULL	IL-6R	GP	level of;;soluble;;CSF	is related to					paranoid-hallucinatory symptoms	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand, a significant relationship between the soluble IL-6R levels in the CSF and the paranoid-hallucinatory symptoms in schizophrenia have been reported (Müller et al., 1997a).	topic_sch
77068	2	356088	5	NULL	NULL	0	NULL	statement 1	Process		occurs in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand, a significant relationship between the soluble IL-6R levels in the CSF and the paranoid-hallucinatory symptoms in schizophrenia have been reported (Müller et al., 1997a).	topic_sch
77069	1	356089	5	NULL	NULL	0	NULL	IL-6	GP		is a product of					monocytes	Cell	active			NULL		0	NULL	NULL	NULL	NULL	NULL	IL-6 is a product of activated monocytes and some authors refer it as a marker of the type-2 immune response, although it is acting as a pro-inflammatory cytokine, too.	topic_sch
77070	2	356089	5	NULL	NULL	0	NULL	IL-6	GP		is a marker of					type-2 immune response	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	IL-6 is a product of activated monocytes and some authors refer it as a marker of the type-2 immune response, although it is acting as a pro-inflammatory cytokine, too.	topic_sch
77071	3	356089	5	NULL	NULL	0	NULL	IL-6	GP		act as					pro-inflammatory cytokine	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	IL-6 is a product of activated monocytes and some authors refer it as a marker of the type-2 immune response, although it is acting as a pro-inflammatory cytokine, too.	topic_sch
77072	1	356090	5	NULL	NULL	0	NULL	type-1 response	Process		is found in		primarily			schizophrenia	MedicalFinding	early stages of			NULL		0	NULL	NULL	NULL	NULL	NULL	It can be hypothesized that the blunted type-1 response is found primarily in early stages of schizophrenia, while a chronic pro-inflammatory stage with an overweight of the type-2 response including high IL-6 levels may predominate in later stages.	topic_sch
77073	2	356090	5	NULL	NULL	0	NULL	pro-inflammatory stage	Time	chronic	occurs along with					type-2 response	Process	overweight of			NULL		0	NULL	NULL	NULL	NULL	NULL	It can be hypothesized that the blunted type-1 response is found primarily in early stages of schizophrenia, while a chronic pro-inflammatory stage with an overweight of the type-2 response including high IL-6 levels may predominate in later stages.	topic_sch
77074	3	356090	5	NULL	NULL	0	NULL	statement 2	Process		includes					IL-6	GP	high levels of			NULL		0	NULL	NULL	NULL	NULL	NULL	It can be hypothesized that the blunted type-1 response is found primarily in early stages of schizophrenia, while a chronic pro-inflammatory stage with an overweight of the type-2 response including high IL-6 levels may predominate in later stages.	topic_sch
77075	4	356090	5	NULL	NULL	0	NULL	statement 3	Process		predominate in					schizophrenia	MedicalFinding	later stages of			NULL		0	NULL	NULL	NULL	NULL	NULL	It can be hypothesized that the blunted type-1 response is found primarily in early stages of schizophrenia, while a chronic pro-inflammatory stage with an overweight of the type-2 response including high IL-6 levels may predominate in later stages.	topic_sch
77076	1	356092	5	NULL	NULL	0	NULL	cyclo-oxygenase-2 inhibitors	Chemical		have therapeutic effects in					schizophrenia	MedicalFinding	early stages of			NULL		0	NULL	NULL	NULL	NULL	NULL	The view of different immune stages can also be underlined from the view of therapeutic studies: as it is discussed later, cyclo-oxygenase-2 inhibitors have therapeutic effects in early stages of schizophrenia, but seemingly only marginal effects in late stages.	topic_sch
77077	2	356092	5	NULL	NULL	0	NULL	cyclo-oxygenase-2 inhibitors	Chemical		effects		marginal			schizophrenia	MedicalFinding	later stages of			NULL		0	NULL	NULL	NULL	NULL	NULL	The view of different immune stages can also be underlined from the view of therapeutic studies: as it is discussed later, cyclo-oxygenase-2 inhibitors have therapeutic effects in early stages of schizophrenia, but seemingly only marginal effects in late stages.	topic_sch
77078	1	356093	5	NULL	NULL	NULL	NULL	 IL-18	GP	levels of;;serum	is elevated in					schizophrenics	GroupOfPeople	medicated			NULL		NULL	NULL	NULL	NULL	NULL	NULL	An elevation of IL-18 serum levels was described in medicated schizophrenics (Tanaka et al., 2000). Since IL-18 plays a pivotal role in the type-1 immune response, this finding is consistent with other descriptions of type-1 activation during antipsychotic treatment.	topic_sch
77079	2	356093	5	NULL	NULL	0	NULL	IL-18	GP		plays a role in		pivotal			type-1 immune response	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	An elevation of IL-18 serum levels was described in medicated schizophrenics (Tanaka et al., 2000). Since IL-18 plays a pivotal role in the type-1 immune response, this finding is consistent with other descriptions of type-1 activation during antipsychotic treatment.	topic_sch
77080	3	356093	5	NULL	NULL	0	NULL	type-1 response	Process		is activated during					antipsychotic treatment	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	An elevation of IL-18 serum levels was described in medicated schizophrenics (Tanaka et al., 2000). Since IL-18 plays a pivotal role in the type-1 immune response, this finding is consistent with other descriptions of type-1 activation during antipsychotic treatment.	topic_sch
77081	1	356094	5	NULL	NULL	NULL	NULL	memory cells	Cell	increase of	is a source of		main			IFN-gamma	GP	production of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	An increase of ‘memory cells’ (CD4+CD45RO+ cells) - one of the main sources of IFN-gamma production - during anti-psychotic therapy with neuroleptics was observed by different groups (Müller et al., 1997c).	topic_sch
77082	2	356094	5	NULL	NULL	0	NULL	neuroleptics	Chemical		is used in					anti-psychotic therapy	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	An increase of ‘memory cells’ (CD4+CD45RO+ cells) - one of the main sources of IFN-gamma production - during anti-psychotic therapy with neuroleptics was observed by different groups (Müller et al., 1997c).	topic_sch
77083	3	356094	5	NULL	NULL	NULL	NULL	memory cells	Cell	increase of	occurs during					statement 2	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	An increase of ‘memory cells’ (CD4+CD45RO+ cells) - one of the main sources of IFN-gamma production - during anti-psychotic therapy with neuroleptics was observed by different groups (Müller et al., 1997c).	topic_sch
77084	1	356095	5	NULL	NULL	0	NULL	sIL-2R	GP	increase in	reflects					IL-2 bearing T-cells	Cell	 increase of;;activated			NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally, an increase of sIL-2R - the increase reflects an increase of activated, IL-2 bearing T-cells - during anti-psychotic treatment was described (Müller et al., 1997b).	topic_sch
77085	2	356095	5	NULL	NULL	0	NULL	statement 1	Process		occurs during					anti-psychotic treatment	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally, an increase of sIL-2R - the increase reflects an increase of activated, IL-2 bearing T-cells - during anti-psychotic treatment was described (Müller et al., 1997b).	topic_sch
77086	1	356096	5	NULL	NULL	0	NULL	sICAM-1	GP	reduced	is increased during		significantly			anti-psychotic therapy	MedicalProcedure	short term			NULL		0	NULL	NULL	NULL	NULL	NULL	The reduced sICAM-1 levels show a significant increase during short term anti-psychotic therapy (Schwarz et al., 2000) and the ICAM-1 ligand leucocyte function antigen-1 (LFA-1) shows a significantly increased expression during antipsychotic therapy (Müller et al., 1999).	topic_sch
77087	2	356096	5	NULL	NULL	0	NULL	ICAM-1 ligand leucocyte function antigen-1	GP	expression of	is increased during		significantly			antipsychotic therapy	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	The reduced sICAM-1 levels show a significant increase during short term anti-psychotic therapy (Schwarz et al., 2000) and the ICAM-1 ligand leucocyte function antigen-1 (LFA-1) shows a significantly increased expression during antipsychotic therapy (Müller et al., 1999).	topic_sch
77088	1	356097	5	NULL	NULL	0	NULL	clozapine tharapy	MedicalProcedure		increases		repeatedly			TNF-alpha	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The increase of TNF-alpha and TNF-alpha receptors during therapy with clozapine was observed repeatedly (Pollmächer et al., 2001).	topic_sch
77089	2	356097	5	NULL	NULL	0	NULL	clozapine tharapy	MedicalProcedure		increases		repeatedly			TNF-alpha receptors	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The increase of TNF-alpha and TNF-alpha receptors during therapy with clozapine was observed repeatedly (Pollmächer et al., 2001).	topic_sch
77343	1	356099	5	NULL	NULL	0	NULL	anti-psychotic therapy	MedicalProcedure		is accompanied by					IL-6	GP	functional decrease of			NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding the type-2 response, several studies point out that anti-psychotic therapy is accompanied by a functional decrease of the IL-6 system (Maes et al., 1997; Müller et al., 2000). These findings provide further evidence that antipsychotics have a ‘balancing’ effect on cytokines.	topic_sch
77344	2	356099	5	NULL	NULL	0	NULL	antipsychotics	Chemical		balancing effect on					cytokines	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding the type-2 response, several studies point out that anti-psychotic therapy is accompanied by a functional decrease of the IL-6 system (Maes et al., 1997; Müller et al., 2000). These findings provide further evidence that antipsychotics have a ‘balancing’ effect on cytokines.	topic_sch
77345	1	356100	5	NULL	NULL	0	NULL	chromosome 7q	Chromosome		undergo					duplication	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Among the discoveries was a duplication in the tip of chromosome 7q. This duplication was found in people with schizophrenia at a rate 14 times that of healthy people. The duplication affects a particular gene called the vasoactive intestinal peptide receptor 2 gene, which is known to play a role in behavior and learning. In people with schizophrenia, the expression of this gene is much higher, the researchers found. The VIPR2 gene mutation, therefore, will be an important target in developing medications that might alter the symptoms of the illness.	topic_sch
77346	2	356100	5	NULL	NULL	0	NULL	statement 1	Process		is found in					people	GroupOfPeople	healthy			NULL		0	NULL	NULL	NULL	NULL	NULL	Among the discoveries was a duplication in the tip of chromosome 7q. This duplication was found in people with schizophrenia at a rate 14 times that of healthy people. The duplication affects a particular gene called the vasoactive intestinal peptide receptor 2 gene, which is known to play a role in behavior and learning. In people with schizophrenia, the expression of this gene is much higher, the researchers found. The VIPR2 gene mutation, therefore, will be an important target in developing medications that might alter the symptoms of the illness.	topic_sch
77347	3	356100	5	NULL	NULL	NULL	NULL	statement 1	Process		is found in					schizophrenic	GroupOfPeople				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Among the discoveries was a duplication in the tip of chromosome 7q. This duplication was found in people with schizophrenia at a rate 14 times that of healthy people. The duplication affects a particular gene called the vasoactive intestinal peptide receptor 2 gene, which is known to play a role in behavior and learning. In people with schizophrenia, the expression of this gene is much higher, the researchers found. The VIPR2 gene mutation, therefore, will be an important target in developing medications that might alter the symptoms of the illness.	topic_sch
77348	4	356100	5	NULL	NULL	0	NULL	statement 3	Process	rate of	is more than					statement 2	Process	rate of			NULL		0	NULL	NULL	NULL	NULL	NULL	Among the discoveries was a duplication in the tip of chromosome 7q. This duplication was found in people with schizophrenia at a rate 14 times that of healthy people. The duplication affects a particular gene called the vasoactive intestinal peptide receptor 2 gene, which is known to play a role in behavior and learning. In people with schizophrenia, the expression of this gene is much higher, the researchers found. The VIPR2 gene mutation, therefore, will be an important target in developing medications that might alter the symptoms of the illness.	topic_sch
77349	5	356100	5	NULL	NULL	0	NULL	statement 1	Process		affects					vasoactive intestinal peptide receptor 2 gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Among the discoveries was a duplication in the tip of chromosome 7q. This duplication was found in people with schizophrenia at a rate 14 times that of healthy people. The duplication affects a particular gene called the vasoactive intestinal peptide receptor 2 gene, which is known to play a role in behavior and learning. In people with schizophrenia, the expression of this gene is much higher, the researchers found. The VIPR2 gene mutation, therefore, will be an important target in developing medications that might alter the symptoms of the illness.	topic_sch
77350	6	356100	5	NULL	NULL	0	NULL	vasoactive intestinal peptide receptor 2 gene	GP		plays a role in					behavior	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Among the discoveries was a duplication in the tip of chromosome 7q. This duplication was found in people with schizophrenia at a rate 14 times that of healthy people. The duplication affects a particular gene called the vasoactive intestinal peptide receptor 2 gene, which is known to play a role in behavior and learning. In people with schizophrenia, the expression of this gene is much higher, the researchers found. The VIPR2 gene mutation, therefore, will be an important target in developing medications that might alter the symptoms of the illness.	topic_sch
77351	7	356100	5	NULL	NULL	0	NULL	vasoactive intestinal peptide receptor 2 gene	GP		plays a role in					learning	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Among the discoveries was a duplication in the tip of chromosome 7q. This duplication was found in people with schizophrenia at a rate 14 times that of healthy people. The duplication affects a particular gene called the vasoactive intestinal peptide receptor 2 gene, which is known to play a role in behavior and learning. In people with schizophrenia, the expression of this gene is much higher, the researchers found. The VIPR2 gene mutation, therefore, will be an important target in developing medications that might alter the symptoms of the illness.	topic_sch
77352	8	356100	5	NULL	NULL	0	NULL	vasoactive intestinal peptide receptor 2 gene	GP		expressed in		highly			schizophrenic	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Among the discoveries was a duplication in the tip of chromosome 7q. This duplication was found in people with schizophrenia at a rate 14 times that of healthy people. The duplication affects a particular gene called the vasoactive intestinal peptide receptor 2 gene, which is known to play a role in behavior and learning. In people with schizophrenia, the expression of this gene is much higher, the researchers found. The VIPR2 gene mutation, therefore, will be an important target in developing medications that might alter the symptoms of the illness.	topic_sch
77353	9	356100	5	NULL	NULL	0	NULL	VIPR2 gene	GP	mutation of	is targeted for					medications	MedicalProcedure	development of			NULL		0	NULL	NULL	NULL	NULL	NULL	Among the discoveries was a duplication in the tip of chromosome 7q. This duplication was found in people with schizophrenia at a rate 14 times that of healthy people. The duplication affects a particular gene called the vasoactive intestinal peptide receptor 2 gene, which is known to play a role in behavior and learning. In people with schizophrenia, the expression of this gene is much higher, the researchers found. The VIPR2 gene mutation, therefore, will be an important target in developing medications that might alter the symptoms of the illness.	topic_sch
77354	10	356100	5	NULL	NULL	0	NULL	statement 9	Process		alter		might			schizophrenia	MedicalFinding	symptoms of			NULL		0	NULL	NULL	NULL	NULL	NULL	Among the discoveries was a duplication in the tip of chromosome 7q. This duplication was found in people with schizophrenia at a rate 14 times that of healthy people. The duplication affects a particular gene called the vasoactive intestinal peptide receptor 2 gene, which is known to play a role in behavior and learning. In people with schizophrenia, the expression of this gene is much higher, the researchers found. The VIPR2 gene mutation, therefore, will be an important target in developing medications that might alter the symptoms of the illness.	topic_sch
77355	1	356101	5	NULL	NULL	0	NULL	energy drinks	Food	caffeinated	trigger					psychotic episode	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Caffeinated energy drinks may trigger a psychotic episode in people with mental illness, an expert has warned after documenting the case of a young man with schizophrenia.	topic_sch
77356	2	356101	5	NULL	NULL	0	NULL	statement 1	Process		occurs in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Caffeinated energy drinks may trigger a psychotic episode in people with mental illness, an expert has warned after documenting the case of a young man with schizophrenia.	topic_sch
77357	1	356102	5	NULL	NULL	0	NULL	antipsychotic drugs	Chemical	use of	treats					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The use of antipsychotic drugs to treat schizophrenia is associated with the loss of a small but measurable amount of brain tissue, a new study finds.	topic_sch
77358	2	356102	5	NULL	NULL	0	NULL	statement 1	Process		is associated with					brain tissue	OrganismPart	loss of;;small;;measurable amount of			NULL		0	NULL	NULL	NULL	NULL	NULL	The use of antipsychotic drugs to treat schizophrenia is associated with the loss of a small but measurable amount of brain tissue, a new study finds.	topic_sch
77359	1	356103	5	NULL	NULL	0	NULL	Creative folks	GroupOfPeople		tend to have					default network	OrganismPart	overactive			NULL		0	NULL	NULL	NULL	NULL	NULL	Creative folks and those with schizophrenia tend to have an overactive default network. 	topic_sch
77360	2	356103	5	NULL	NULL	NULL	NULL	Schizophrenic people	GroupOfPeople		tend to have					default network	OrganismPart	overactive			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Creative folks and those with schizophrenia tend to have an overactive default network. 	topic_sch
77361	1	356104	5	NULL	NULL	NULL	NULL	brain network	OrganismPart		involves					working memory network	OrganismPart				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Research shows that when most of us fall asleep, the brain network that involves attention to the outside world (the working memory network consisting primarily of the lateral frontal and parietal cortices) deactivates and our default brain network (medial prefrontal and posterior cingulate cortices) takes over. The discovery of the default brain network is important, as it involves various aspects of our self, such as our self-representations, dreams, imagination, current concerns, autobiographical memory and perspective-taking ability. Those with higher default network activity during rest have a tendency to daydream more frequently, which makes sense if one thinks of the default network as involving our inner stream of consciousness.	topic_sch
77362	2	356104	5	NULL	NULL	0	NULL	brain network	OrganismPart		involves					default brain network	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Research shows that when most of us fall asleep, the brain network that involves attention to the outside world (the working memory network consisting primarily of the lateral frontal and parietal cortices) deactivates and our default brain network (medial prefrontal and posterior cingulate cortices) takes over. The discovery of the default brain network is important, as it involves various aspects of our self, such as our self-representations, dreams, imagination, current concerns, autobiographical memory and perspective-taking ability. Those with higher default network activity during rest have a tendency to daydream more frequently, which makes sense if one thinks of the default network as involving our inner stream of consciousness.	topic_sch
77363	3	356104	5	NULL	NULL	0	NULL	statement 1	Process		occurs along with					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Research shows that when most of us fall asleep, the brain network that involves attention to the outside world (the working memory network consisting primarily of the lateral frontal and parietal cortices) deactivates and our default brain network (medial prefrontal and posterior cingulate cortices) takes over. The discovery of the default brain network is important, as it involves various aspects of our self, such as our self-representations, dreams, imagination, current concerns, autobiographical memory and perspective-taking ability. Those with higher default network activity during rest have a tendency to daydream more frequently, which makes sense if one thinks of the default network as involving our inner stream of consciousness.	topic_sch
77364	4	356104	5	NULL	NULL	0	NULL	world	GeographicNotProper	attention to;;outside	is known as					 working memory network	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Research shows that when most of us fall asleep, the brain network that involves attention to the outside world (the working memory network consisting primarily of the lateral frontal and parietal cortices) deactivates and our default brain network (medial prefrontal and posterior cingulate cortices) takes over. The discovery of the default brain network is important, as it involves various aspects of our self, such as our self-representations, dreams, imagination, current concerns, autobiographical memory and perspective-taking ability. Those with higher default network activity during rest have a tendency to daydream more frequently, which makes sense if one thinks of the default network as involving our inner stream of consciousness.	topic_sch
77365	5	356104	5	NULL	NULL	0	NULL	working memory network	OrganismPart		consists of		primarily			lateral cortex	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Research shows that when most of us fall asleep, the brain network that involves attention to the outside world (the working memory network consisting primarily of the lateral frontal and parietal cortices) deactivates and our default brain network (medial prefrontal and posterior cingulate cortices) takes over. The discovery of the default brain network is important, as it involves various aspects of our self, such as our self-representations, dreams, imagination, current concerns, autobiographical memory and perspective-taking ability. Those with higher default network activity during rest have a tendency to daydream more frequently, which makes sense if one thinks of the default network as involving our inner stream of consciousness.	topic_sch
77366	6	356104	5	NULL	NULL	0	NULL	working memory network	OrganismPart		consists of		primarily			frontal cortex	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Research shows that when most of us fall asleep, the brain network that involves attention to the outside world (the working memory network consisting primarily of the lateral frontal and parietal cortices) deactivates and our default brain network (medial prefrontal and posterior cingulate cortices) takes over. The discovery of the default brain network is important, as it involves various aspects of our self, such as our self-representations, dreams, imagination, current concerns, autobiographical memory and perspective-taking ability. Those with higher default network activity during rest have a tendency to daydream more frequently, which makes sense if one thinks of the default network as involving our inner stream of consciousness.	topic_sch
77367	7	356104	5	NULL	NULL	0	NULL	working memory network	OrganismPart		consists of		primarily			parietal cortex	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Research shows that when most of us fall asleep, the brain network that involves attention to the outside world (the working memory network consisting primarily of the lateral frontal and parietal cortices) deactivates and our default brain network (medial prefrontal and posterior cingulate cortices) takes over. The discovery of the default brain network is important, as it involves various aspects of our self, such as our self-representations, dreams, imagination, current concerns, autobiographical memory and perspective-taking ability. Those with higher default network activity during rest have a tendency to daydream more frequently, which makes sense if one thinks of the default network as involving our inner stream of consciousness.	topic_sch
77368	8	356104	5	NULL	NULL	0	NULL	default brain network	OrganismPart		consists of					medial prefrontal cortex	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Research shows that when most of us fall asleep, the brain network that involves attention to the outside world (the working memory network consisting primarily of the lateral frontal and parietal cortices) deactivates and our default brain network (medial prefrontal and posterior cingulate cortices) takes over. The discovery of the default brain network is important, as it involves various aspects of our self, such as our self-representations, dreams, imagination, current concerns, autobiographical memory and perspective-taking ability. Those with higher default network activity during rest have a tendency to daydream more frequently, which makes sense if one thinks of the default network as involving our inner stream of consciousness.	topic_sch
77369	9	356104	5	NULL	NULL	0	NULL	default brain network	OrganismPart		consists of					posterior cingulate cortex	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Research shows that when most of us fall asleep, the brain network that involves attention to the outside world (the working memory network consisting primarily of the lateral frontal and parietal cortices) deactivates and our default brain network (medial prefrontal and posterior cingulate cortices) takes over. The discovery of the default brain network is important, as it involves various aspects of our self, such as our self-representations, dreams, imagination, current concerns, autobiographical memory and perspective-taking ability. Those with higher default network activity during rest have a tendency to daydream more frequently, which makes sense if one thinks of the default network as involving our inner stream of consciousness.	topic_sch
77370	10	356104	5	NULL	NULL	0	NULL	working memory network	OrganismPart	deactivation of	is followed by					default network	OrganismPart	taking over of			NULL		0	NULL	NULL	NULL	NULL	NULL	Research shows that when most of us fall asleep, the brain network that involves attention to the outside world (the working memory network consisting primarily of the lateral frontal and parietal cortices) deactivates and our default brain network (medial prefrontal and posterior cingulate cortices) takes over. The discovery of the default brain network is important, as it involves various aspects of our self, such as our self-representations, dreams, imagination, current concerns, autobiographical memory and perspective-taking ability. Those with higher default network activity during rest have a tendency to daydream more frequently, which makes sense if one thinks of the default network as involving our inner stream of consciousness.	topic_sch
77371	11	356104	5	NULL	NULL	0	NULL	statement 10	Process		occurs during					sleep	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Research shows that when most of us fall asleep, the brain network that involves attention to the outside world (the working memory network consisting primarily of the lateral frontal and parietal cortices) deactivates and our default brain network (medial prefrontal and posterior cingulate cortices) takes over. The discovery of the default brain network is important, as it involves various aspects of our self, such as our self-representations, dreams, imagination, current concerns, autobiographical memory and perspective-taking ability. Those with higher default network activity during rest have a tendency to daydream more frequently, which makes sense if one thinks of the default network as involving our inner stream of consciousness.	topic_sch
77372	12	356104	5	NULL	NULL	0	NULL	default brain network	OrganismPart		involves					self-representations	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Research shows that when most of us fall asleep, the brain network that involves attention to the outside world (the working memory network consisting primarily of the lateral frontal and parietal cortices) deactivates and our default brain network (medial prefrontal and posterior cingulate cortices) takes over. The discovery of the default brain network is important, as it involves various aspects of our self, such as our self-representations, dreams, imagination, current concerns, autobiographical memory and perspective-taking ability. Those with higher default network activity during rest have a tendency to daydream more frequently, which makes sense if one thinks of the default network as involving our inner stream of consciousness.	topic_sch
77373	13	356104	5	NULL	NULL	0	NULL	default brain network	OrganismPart		involves					dreams	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Research shows that when most of us fall asleep, the brain network that involves attention to the outside world (the working memory network consisting primarily of the lateral frontal and parietal cortices) deactivates and our default brain network (medial prefrontal and posterior cingulate cortices) takes over. The discovery of the default brain network is important, as it involves various aspects of our self, such as our self-representations, dreams, imagination, current concerns, autobiographical memory and perspective-taking ability. Those with higher default network activity during rest have a tendency to daydream more frequently, which makes sense if one thinks of the default network as involving our inner stream of consciousness.	topic_sch
77374	14	356104	5	NULL	NULL	0	NULL	default brain network	OrganismPart		involves					imagination	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Research shows that when most of us fall asleep, the brain network that involves attention to the outside world (the working memory network consisting primarily of the lateral frontal and parietal cortices) deactivates and our default brain network (medial prefrontal and posterior cingulate cortices) takes over. The discovery of the default brain network is important, as it involves various aspects of our self, such as our self-representations, dreams, imagination, current concerns, autobiographical memory and perspective-taking ability. Those with higher default network activity during rest have a tendency to daydream more frequently, which makes sense if one thinks of the default network as involving our inner stream of consciousness.	topic_sch
77375	15	356104	5	NULL	NULL	0	NULL	default brain network	OrganismPart		involves					current concerns	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Research shows that when most of us fall asleep, the brain network that involves attention to the outside world (the working memory network consisting primarily of the lateral frontal and parietal cortices) deactivates and our default brain network (medial prefrontal and posterior cingulate cortices) takes over. The discovery of the default brain network is important, as it involves various aspects of our self, such as our self-representations, dreams, imagination, current concerns, autobiographical memory and perspective-taking ability. Those with higher default network activity during rest have a tendency to daydream more frequently, which makes sense if one thinks of the default network as involving our inner stream of consciousness.	topic_sch
77376	16	356104	5	NULL	NULL	0	NULL	default brain network	OrganismPart		involves					autobiographical memory	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Research shows that when most of us fall asleep, the brain network that involves attention to the outside world (the working memory network consisting primarily of the lateral frontal and parietal cortices) deactivates and our default brain network (medial prefrontal and posterior cingulate cortices) takes over. The discovery of the default brain network is important, as it involves various aspects of our self, such as our self-representations, dreams, imagination, current concerns, autobiographical memory and perspective-taking ability. Those with higher default network activity during rest have a tendency to daydream more frequently, which makes sense if one thinks of the default network as involving our inner stream of consciousness.	topic_sch
77377	17	356104	5	NULL	NULL	0	NULL	default brain network	OrganismPart		involves					perspective-taking ability	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Research shows that when most of us fall asleep, the brain network that involves attention to the outside world (the working memory network consisting primarily of the lateral frontal and parietal cortices) deactivates and our default brain network (medial prefrontal and posterior cingulate cortices) takes over. The discovery of the default brain network is important, as it involves various aspects of our self, such as our self-representations, dreams, imagination, current concerns, autobiographical memory and perspective-taking ability. Those with higher default network activity during rest have a tendency to daydream more frequently, which makes sense if one thinks of the default network as involving our inner stream of consciousness.	topic_sch
77378	18	356104	5	NULL	NULL	0	NULL	people	GroupOfPeople		have					default network activity	Process	higher			NULL		0	NULL	NULL	NULL	NULL	NULL	Research shows that when most of us fall asleep, the brain network that involves attention to the outside world (the working memory network consisting primarily of the lateral frontal and parietal cortices) deactivates and our default brain network (medial prefrontal and posterior cingulate cortices) takes over. The discovery of the default brain network is important, as it involves various aspects of our self, such as our self-representations, dreams, imagination, current concerns, autobiographical memory and perspective-taking ability. Those with higher default network activity during rest have a tendency to daydream more frequently, which makes sense if one thinks of the default network as involving our inner stream of consciousness.	topic_sch
77379	19	356104	5	NULL	NULL	0	NULL	statement 18	Process		occurs during					rest	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Research shows that when most of us fall asleep, the brain network that involves attention to the outside world (the working memory network consisting primarily of the lateral frontal and parietal cortices) deactivates and our default brain network (medial prefrontal and posterior cingulate cortices) takes over. The discovery of the default brain network is important, as it involves various aspects of our self, such as our self-representations, dreams, imagination, current concerns, autobiographical memory and perspective-taking ability. Those with higher default network activity during rest have a tendency to daydream more frequently, which makes sense if one thinks of the default network as involving our inner stream of consciousness.	topic_sch
77380	20	356104	5	NULL	NULL	NULL	NULL	statement 18	Process		tendency to		frequently			daydream	MentalProcess				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Research shows that when most of us fall asleep, the brain network that involves attention to the outside world (the working memory network consisting primarily of the lateral frontal and parietal cortices) deactivates and our default brain network (medial prefrontal and posterior cingulate cortices) takes over. The discovery of the default brain network is important, as it involves various aspects of our self, such as our self-representations, dreams, imagination, current concerns, autobiographical memory and perspective-taking ability. Those with higher default network activity during rest have a tendency to daydream more frequently, which makes sense if one thinks of the default network as involving our inner stream of consciousness.	topic_sch
77381	21	356104	5	NULL	NULL	0	NULL	default network	OrganismPart		involves					consciousness	MentalProcess	inner stream of			NULL		0	NULL	NULL	NULL	NULL	NULL	Research shows that when most of us fall asleep, the brain network that involves attention to the outside world (the working memory network consisting primarily of the lateral frontal and parietal cortices) deactivates and our default brain network (medial prefrontal and posterior cingulate cortices) takes over. The discovery of the default brain network is important, as it involves various aspects of our self, such as our self-representations, dreams, imagination, current concerns, autobiographical memory and perspective-taking ability. Those with higher default network activity during rest have a tendency to daydream more frequently, which makes sense if one thinks of the default network as involving our inner stream of consciousness.	topic_sch
77634	1	356107	7	NULL	NULL	0	NULL	valproic acid	Chemical		role for					BPD	MedicalFinding	epigenetic mechanism in			NULL		0	NULL	NULL	NULL	NULL	NULL	valproic acid introduced a role for epigenetic mechanisms in BPD	topic_bd
77635	1	356108	7	NULL	NULL	0	NULL	lithium 	Chemical	studies with	led to the					glycogen synthase kinase 3 beta pathway	Process	hypothesis of a role of			NULL		0	NULL	NULL	NULL	NULL	NULL	Discovery-driven studies and novel technologies changed that picture and created interesting new models. Initial studies focused on known neurotransmitter systems such as biogenic amines ([Cousins et al., 2009], [Manji and Lenox, 2000] and [Schildkraut, 1974]), glutamate, and GABA ([Krystal et al., 2002] and Post, 1990 R.M. Post, Non-lithium treatment for bipolar disorder, J. Clin. Psychiatry 51 (Suppl) (1990), pp. 9–16 discussion 17–9. View Record in Scopus | Cited By in Scopus (37)[Post, 1990]), and on altered regulation of glucocorticoids ([Daban et al., 2005] and [Watson et al., 2004]), with implications of an involvement of each system. Studies with lithium led to the hypothesis of a role of the glycogen synthase kinase 3 beta pathway ([Ikonomov and Manji, 1999] and [Klein and Melton, 1996]), while studies with valproic acid introduced a role for epigenetic mechanisms in BPD (Phiel et al., 2001). Serotonin and norepinephrine became a focus because of their involvement in the mechanism of action of antidepressants (Owens, 2004). Overall, many different systems seemed to be implicated in BPD, with supportive evidence for each one.	topic_bd
77636	2	356108	7	NULL	NULL	0	NULL	statement 1	Process		occur in					BPD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Discovery-driven studies and novel technologies changed that picture and created interesting new models. Initial studies focused on known neurotransmitter systems such as biogenic amines ([Cousins et al., 2009], [Manji and Lenox, 2000] and [Schildkraut, 1974]), glutamate, and GABA ([Krystal et al., 2002] and Post, 1990 R.M. Post, Non-lithium treatment for bipolar disorder, J. Clin. Psychiatry 51 (Suppl) (1990), pp. 9–16 discussion 17–9. View Record in Scopus | Cited By in Scopus (37)[Post, 1990]), and on altered regulation of glucocorticoids ([Daban et al., 2005] and [Watson et al., 2004]), with implications of an involvement of each system. Studies with lithium led to the hypothesis of a role of the glycogen synthase kinase 3 beta pathway ([Ikonomov and Manji, 1999] and [Klein and Melton, 1996]), while studies with valproic acid introduced a role for epigenetic mechanisms in BPD (Phiel et al., 2001). Serotonin and norepinephrine became a focus because of their involvement in the mechanism of action of antidepressants (Owens, 2004). Overall, many different systems seemed to be implicated in BPD, with supportive evidence for each one.	topic_bd
77637	3	356108	7	NULL	NULL	0	NULL	 valproic acid	Chemical	studies with	introduced a					epigenetic mechanism	Process	role for			NULL		0	NULL	NULL	NULL	NULL	NULL	Discovery-driven studies and novel technologies changed that picture and created interesting new models. Initial studies focused on known neurotransmitter systems such as biogenic amines ([Cousins et al., 2009], [Manji and Lenox, 2000] and [Schildkraut, 1974]), glutamate, and GABA ([Krystal et al., 2002] and Post, 1990 R.M. Post, Non-lithium treatment for bipolar disorder, J. Clin. Psychiatry 51 (Suppl) (1990), pp. 9–16 discussion 17–9. View Record in Scopus | Cited By in Scopus (37)[Post, 1990]), and on altered regulation of glucocorticoids ([Daban et al., 2005] and [Watson et al., 2004]), with implications of an involvement of each system. Studies with lithium led to the hypothesis of a role of the glycogen synthase kinase 3 beta pathway ([Ikonomov and Manji, 1999] and [Klein and Melton, 1996]), while studies with valproic acid introduced a role for epigenetic mechanisms in BPD (Phiel et al., 2001). Serotonin and norepinephrine became a focus because of their involvement in the mechanism of action of antidepressants (Owens, 2004). Overall, many different systems seemed to be implicated in BPD, with supportive evidence for each one.	topic_bd
77638	4	356108	7	NULL	NULL	0	NULL	statement 3	Process		occur in					BPD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Discovery-driven studies and novel technologies changed that picture and created interesting new models. Initial studies focused on known neurotransmitter systems such as biogenic amines ([Cousins et al., 2009], [Manji and Lenox, 2000] and [Schildkraut, 1974]), glutamate, and GABA ([Krystal et al., 2002] and Post, 1990 R.M. Post, Non-lithium treatment for bipolar disorder, J. Clin. Psychiatry 51 (Suppl) (1990), pp. 9–16 discussion 17–9. View Record in Scopus | Cited By in Scopus (37)[Post, 1990]), and on altered regulation of glucocorticoids ([Daban et al., 2005] and [Watson et al., 2004]), with implications of an involvement of each system. Studies with lithium led to the hypothesis of a role of the glycogen synthase kinase 3 beta pathway ([Ikonomov and Manji, 1999] and [Klein and Melton, 1996]), while studies with valproic acid introduced a role for epigenetic mechanisms in BPD (Phiel et al., 2001). Serotonin and norepinephrine became a focus because of their involvement in the mechanism of action of antidepressants (Owens, 2004). Overall, many different systems seemed to be implicated in BPD, with supportive evidence for each one.	topic_bd
77639	5	356108	7	NULL	NULL	0	NULL	serotonin	Chemical		is involved in					antidepressant 	Chemical	mechanism of;;action of			NULL		0	NULL	NULL	NULL	NULL	NULL	Discovery-driven studies and novel technologies changed that picture and created interesting new models. Initial studies focused on known neurotransmitter systems such as biogenic amines ([Cousins et al., 2009], [Manji and Lenox, 2000] and [Schildkraut, 1974]), glutamate, and GABA ([Krystal et al., 2002] and Post, 1990 R.M. Post, Non-lithium treatment for bipolar disorder, J. Clin. Psychiatry 51 (Suppl) (1990), pp. 9–16 discussion 17–9. View Record in Scopus | Cited By in Scopus (37)[Post, 1990]), and on altered regulation of glucocorticoids ([Daban et al., 2005] and [Watson et al., 2004]), with implications of an involvement of each system. Studies with lithium led to the hypothesis of a role of the glycogen synthase kinase 3 beta pathway ([Ikonomov and Manji, 1999] and [Klein and Melton, 1996]), while studies with valproic acid introduced a role for epigenetic mechanisms in BPD (Phiel et al., 2001). Serotonin and norepinephrine became a focus because of their involvement in the mechanism of action of antidepressants (Owens, 2004). Overall, many different systems seemed to be implicated in BPD, with supportive evidence for each one.	topic_bd
77640	6	356108	7	NULL	NULL	0	NULL	norepinephrine	Chemical		is involved in					antidepressant 	Chemical	mechanism of;;action of			NULL		0	NULL	NULL	NULL	NULL	NULL	Discovery-driven studies and novel technologies changed that picture and created interesting new models. Initial studies focused on known neurotransmitter systems such as biogenic amines ([Cousins et al., 2009], [Manji and Lenox, 2000] and [Schildkraut, 1974]), glutamate, and GABA ([Krystal et al., 2002] and Post, 1990 R.M. Post, Non-lithium treatment for bipolar disorder, J. Clin. Psychiatry 51 (Suppl) (1990), pp. 9–16 discussion 17–9. View Record in Scopus | Cited By in Scopus (37)[Post, 1990]), and on altered regulation of glucocorticoids ([Daban et al., 2005] and [Watson et al., 2004]), with implications of an involvement of each system. Studies with lithium led to the hypothesis of a role of the glycogen synthase kinase 3 beta pathway ([Ikonomov and Manji, 1999] and [Klein and Melton, 1996]), while studies with valproic acid introduced a role for epigenetic mechanisms in BPD (Phiel et al., 2001). Serotonin and norepinephrine became a focus because of their involvement in the mechanism of action of antidepressants (Owens, 2004). Overall, many different systems seemed to be implicated in BPD, with supportive evidence for each one.	topic_bd
77641	1	356109	7	NULL	NULL	0	NULL	GC	Chemical		bind					GR	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Glucocorticoids (GC) are a class of steroid hormones that bind to the glucocorticoid receptor (GR), which is present in almost every vertebrate animal cell	topic_bd
77642	2	356109	7	NULL	NULL	0	NULL	GC	Chemical		is a type of					steroid hormones	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Glucocorticoids (GC) are a class of steroid hormones that bind to the glucocorticoid receptor (GR), which is present in almost every vertebrate animal cell	topic_bd
77643	3	356109	7	NULL	NULL	0	NULL	GR	GP		is					glucocorticoid receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Glucocorticoids (GC) are a class of steroid hormones that bind to the glucocorticoid receptor (GR), which is present in almost every vertebrate animal cell	topic_bd
77644	4	356109	7	NULL	NULL	0	NULL	GR	GP		is present in					vertebrate animal cell	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Glucocorticoids (GC) are a class of steroid hormones that bind to the glucocorticoid receptor (GR), which is present in almost every vertebrate animal cell	topic_bd
77645	1	356110	7	NULL	NULL	0	NULL	Gene expression profile	GP		shows					mRNA	NucleicAcid	decrease of			NULL		0	NULL	NULL	NULL	NULL	NULL	Gene and protein expression profiles in BPD show a decrease of mRNA and proteins involved in mitochondrial functions such as oxidative phosphorylation (OXPHOS)	topic_bd
77646	2	356110	7	NULL	NULL	0	NULL	mRNA	NucleicAcid		involved in					OXPHOS	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Gene and protein expression profiles in BPD show a decrease of mRNA and proteins involved in mitochondrial functions such as oxidative phosphorylation (OXPHOS)	topic_bd
77647	3	356110	7	NULL	NULL	0	NULL	protein expression profile	GP		shows					proteins	GP	decrease of			NULL		0	NULL	NULL	NULL	NULL	NULL	Gene and protein expression profiles in BPD show a decrease of mRNA and proteins involved in mitochondrial functions such as oxidative phosphorylation (OXPHOS)	topic_bd
77648	4	356110	7	NULL	NULL	0	NULL	proteins	GP		involved in					OXPHOS	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Gene and protein expression profiles in BPD show a decrease of mRNA and proteins involved in mitochondrial functions such as oxidative phosphorylation (OXPHOS)	topic_bd
77649	5	356110	7	NULL	NULL	0	NULL	OXPHOS	Process		is					oxidative phosphorylation	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Gene and protein expression profiles in BPD show a decrease of mRNA and proteins involved in mitochondrial functions such as oxidative phosphorylation (OXPHOS)	topic_bd
77650	6	356110	7	NULL	NULL	0	NULL	OXPHOS	Process		is a type of					mitochondrial function	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Gene and protein expression profiles in BPD show a decrease of mRNA and proteins involved in mitochondrial functions such as oxidative phosphorylation (OXPHOS)	topic_bd
77651	1	356111	7	NULL	NULL	0	NULL	Gene expression profile	GP		shows 					mRNA	NucleicAcid	decrease of			NULL		0	NULL	NULL	NULL	NULL	NULL	Gene and protein expression profiles in BPD show a decrease of mRNA and proteins involved in mitochondrial functions such as oxidative phosphorylation (OXPHOS) (Iwamoto et al., 2005 K. Iwamoto, M. Bundo and T. Kato, Altered expression of mitochondria-related genes in postmortem brains of patients with bipolar disorder or schizophrenia, as revealed by large-scale DNA microarray analysis, Hum. Mol. Genet. 14 (2005), pp. 241–253. View Record in Scopus | Cited By in Scopus (130)[Iwamoto et al., 2005], [Konradi et al., 2004], [Pennington et al., 2008] and [Washizuka et al., 2005]). Downregulations were observed in the prefrontal cortex (PFC; Brodmann areas 9 and 46, Table 1), ([Iwamoto et al., 2005], [Pennington et al., 2008] and [Sun et al., 2006]), hippocampus (Konradi et al., 2004) and in lymphoblastoid cell lines (Table 2), (Washizuka et al., 2005). Under compromised OXPHOS, ATP levels decrease and the activity of ATP-dependent ion pumps such as the Na+/K+-ATPase is slowed down, causing the membrane potential to shift toward hypopolarization. Neurotransmitters are released, and their uptake is delayed.	topic_bd
77652	2	356111	7	NULL	NULL	0	NULL	mRNA	NucleicAcid		involved in					OXPHOS	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Gene and protein expression profiles in BPD show a decrease of mRNA and proteins involved in mitochondrial functions such as oxidative phosphorylation (OXPHOS) (Iwamoto et al., 2005 K. Iwamoto, M. Bundo and T. Kato, Altered expression of mitochondria-related genes in postmortem brains of patients with bipolar disorder or schizophrenia, as revealed by large-scale DNA microarray analysis, Hum. Mol. Genet. 14 (2005), pp. 241–253. View Record in Scopus | Cited By in Scopus (130)[Iwamoto et al., 2005], [Konradi et al., 2004], [Pennington et al., 2008] and [Washizuka et al., 2005]). Downregulations were observed in the prefrontal cortex (PFC; Brodmann areas 9 and 46, Table 1), ([Iwamoto et al., 2005], [Pennington et al., 2008] and [Sun et al., 2006]), hippocampus (Konradi et al., 2004) and in lymphoblastoid cell lines (Table 2), (Washizuka et al., 2005). Under compromised OXPHOS, ATP levels decrease and the activity of ATP-dependent ion pumps such as the Na+/K+-ATPase is slowed down, causing the membrane potential to shift toward hypopolarization. Neurotransmitters are released, and their uptake is delayed.	topic_bd
77653	3	356111	7	NULL	NULL	0	NULL	protein expression profile	GP		shows					proteins	GP	decrease of			NULL		0	NULL	NULL	NULL	NULL	NULL	Gene and protein expression profiles in BPD show a decrease of mRNA and proteins involved in mitochondrial functions such as oxidative phosphorylation (OXPHOS) (Iwamoto et al., 2005 K. Iwamoto, M. Bundo and T. Kato, Altered expression of mitochondria-related genes in postmortem brains of patients with bipolar disorder or schizophrenia, as revealed by large-scale DNA microarray analysis, Hum. Mol. Genet. 14 (2005), pp. 241–253. View Record in Scopus | Cited By in Scopus (130)[Iwamoto et al., 2005], [Konradi et al., 2004], [Pennington et al., 2008] and [Washizuka et al., 2005]). Downregulations were observed in the prefrontal cortex (PFC; Brodmann areas 9 and 46, Table 1), ([Iwamoto et al., 2005], [Pennington et al., 2008] and [Sun et al., 2006]), hippocampus (Konradi et al., 2004) and in lymphoblastoid cell lines (Table 2), (Washizuka et al., 2005). Under compromised OXPHOS, ATP levels decrease and the activity of ATP-dependent ion pumps such as the Na+/K+-ATPase is slowed down, causing the membrane potential to shift toward hypopolarization. Neurotransmitters are released, and their uptake is delayed.	topic_bd
77654	4	356111	7	NULL	NULL	0	NULL	proteins	GP		involved in					OXPHOS	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Gene and protein expression profiles in BPD show a decrease of mRNA and proteins involved in mitochondrial functions such as oxidative phosphorylation (OXPHOS) (Iwamoto et al., 2005 K. Iwamoto, M. Bundo and T. Kato, Altered expression of mitochondria-related genes in postmortem brains of patients with bipolar disorder or schizophrenia, as revealed by large-scale DNA microarray analysis, Hum. Mol. Genet. 14 (2005), pp. 241–253. View Record in Scopus | Cited By in Scopus (130)[Iwamoto et al., 2005], [Konradi et al., 2004], [Pennington et al., 2008] and [Washizuka et al., 2005]). Downregulations were observed in the prefrontal cortex (PFC; Brodmann areas 9 and 46, Table 1), ([Iwamoto et al., 2005], [Pennington et al., 2008] and [Sun et al., 2006]), hippocampus (Konradi et al., 2004) and in lymphoblastoid cell lines (Table 2), (Washizuka et al., 2005). Under compromised OXPHOS, ATP levels decrease and the activity of ATP-dependent ion pumps such as the Na+/K+-ATPase is slowed down, causing the membrane potential to shift toward hypopolarization. Neurotransmitters are released, and their uptake is delayed.	topic_bd
77655	5	356111	7	NULL	NULL	0	NULL	OXPHOS	Process		is					oxidative phosphorylation	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Gene and protein expression profiles in BPD show a decrease of mRNA and proteins involved in mitochondrial functions such as oxidative phosphorylation (OXPHOS) (Iwamoto et al., 2005 K. Iwamoto, M. Bundo and T. Kato, Altered expression of mitochondria-related genes in postmortem brains of patients with bipolar disorder or schizophrenia, as revealed by large-scale DNA microarray analysis, Hum. Mol. Genet. 14 (2005), pp. 241–253. View Record in Scopus | Cited By in Scopus (130)[Iwamoto et al., 2005], [Konradi et al., 2004], [Pennington et al., 2008] and [Washizuka et al., 2005]). Downregulations were observed in the prefrontal cortex (PFC; Brodmann areas 9 and 46, Table 1), ([Iwamoto et al., 2005], [Pennington et al., 2008] and [Sun et al., 2006]), hippocampus (Konradi et al., 2004) and in lymphoblastoid cell lines (Table 2), (Washizuka et al., 2005). Under compromised OXPHOS, ATP levels decrease and the activity of ATP-dependent ion pumps such as the Na+/K+-ATPase is slowed down, causing the membrane potential to shift toward hypopolarization. Neurotransmitters are released, and their uptake is delayed.	topic_bd
77656	6	356111	7	NULL	NULL	0	NULL	OXPHOS	Process		is a type of					mitochondrial function	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Gene and protein expression profiles in BPD show a decrease of mRNA and proteins involved in mitochondrial functions such as oxidative phosphorylation (OXPHOS) (Iwamoto et al., 2005 K. Iwamoto, M. Bundo and T. Kato, Altered expression of mitochondria-related genes in postmortem brains of patients with bipolar disorder or schizophrenia, as revealed by large-scale DNA microarray analysis, Hum. Mol. Genet. 14 (2005), pp. 241–253. View Record in Scopus | Cited By in Scopus (130)[Iwamoto et al., 2005], [Konradi et al., 2004], [Pennington et al., 2008] and [Washizuka et al., 2005]). Downregulations were observed in the prefrontal cortex (PFC; Brodmann areas 9 and 46, Table 1), ([Iwamoto et al., 2005], [Pennington et al., 2008] and [Sun et al., 2006]), hippocampus (Konradi et al., 2004) and in lymphoblastoid cell lines (Table 2), (Washizuka et al., 2005). Under compromised OXPHOS, ATP levels decrease and the activity of ATP-dependent ion pumps such as the Na+/K+-ATPase is slowed down, causing the membrane potential to shift toward hypopolarization. Neurotransmitters are released, and their uptake is delayed.	topic_bd
77657	7	356111	7	NULL	NULL	NULL	NULL	mitochondria-related genes	GP	altered expression of	occur in					bipolar disorder	MedicalFinding				NULL	postmortem brains of patients	NULL	NULL	NULL	NULL	NULL	NULL	Gene and protein expression profiles in BPD show a decrease of mRNA and proteins involved in mitochondrial functions such as oxidative phosphorylation (OXPHOS) (Iwamoto et al., 2005 K. Iwamoto, M. Bundo and T. Kato, Altered expression of mitochondria-related genes in postmortem brains of patients with bipolar disorder or schizophrenia, as revealed by large-scale DNA microarray analysis, Hum. Mol. Genet. 14 (2005), pp. 241–253. View Record in Scopus | Cited By in Scopus (130)[Iwamoto et al., 2005], [Konradi et al., 2004], [Pennington et al., 2008] and [Washizuka et al., 2005]). Downregulations were observed in the prefrontal cortex (PFC; Brodmann areas 9 and 46, Table 1), ([Iwamoto et al., 2005], [Pennington et al., 2008] and [Sun et al., 2006]), hippocampus (Konradi et al., 2004) and in lymphoblastoid cell lines (Table 2), (Washizuka et al., 2005). Under compromised OXPHOS, ATP levels decrease and the activity of ATP-dependent ion pumps such as the Na+/K+-ATPase is slowed down, causing the membrane potential to shift toward hypopolarization. Neurotransmitters are released, and their uptake is delayed.	topic_bd
77658	8	356111	7	NULL	NULL	NULL	NULL	mitochondria-related genes	GP	altered expression of	occur in					schizophrenia	MedicalFinding				NULL	postmortem brains of patients	NULL	NULL	NULL	NULL	NULL	NULL	Gene and protein expression profiles in BPD show a decrease of mRNA and proteins involved in mitochondrial functions such as oxidative phosphorylation (OXPHOS) (Iwamoto et al., 2005 K. Iwamoto, M. Bundo and T. Kato, Altered expression of mitochondria-related genes in postmortem brains of patients with bipolar disorder or schizophrenia, as revealed by large-scale DNA microarray analysis, Hum. Mol. Genet. 14 (2005), pp. 241–253. View Record in Scopus | Cited By in Scopus (130)[Iwamoto et al., 2005], [Konradi et al., 2004], [Pennington et al., 2008] and [Washizuka et al., 2005]). Downregulations were observed in the prefrontal cortex (PFC; Brodmann areas 9 and 46, Table 1), ([Iwamoto et al., 2005], [Pennington et al., 2008] and [Sun et al., 2006]), hippocampus (Konradi et al., 2004) and in lymphoblastoid cell lines (Table 2), (Washizuka et al., 2005). Under compromised OXPHOS, ATP levels decrease and the activity of ATP-dependent ion pumps such as the Na+/K+-ATPase is slowed down, causing the membrane potential to shift toward hypopolarization. Neurotransmitters are released, and their uptake is delayed.	topic_bd
77659	9	356111	7	NULL	NULL	0	NULL	ATP	Chemical	levels of	decrease					OXPHOS	Process	under compromised			NULL		0	NULL	NULL	NULL	NULL	NULL	Gene and protein expression profiles in BPD show a decrease of mRNA and proteins involved in mitochondrial functions such as oxidative phosphorylation (OXPHOS) (Iwamoto et al., 2005 K. Iwamoto, M. Bundo and T. Kato, Altered expression of mitochondria-related genes in postmortem brains of patients with bipolar disorder or schizophrenia, as revealed by large-scale DNA microarray analysis, Hum. Mol. Genet. 14 (2005), pp. 241–253. View Record in Scopus | Cited By in Scopus (130)[Iwamoto et al., 2005], [Konradi et al., 2004], [Pennington et al., 2008] and [Washizuka et al., 2005]). Downregulations were observed in the prefrontal cortex (PFC; Brodmann areas 9 and 46, Table 1), ([Iwamoto et al., 2005], [Pennington et al., 2008] and [Sun et al., 2006]), hippocampus (Konradi et al., 2004) and in lymphoblastoid cell lines (Table 2), (Washizuka et al., 2005). Under compromised OXPHOS, ATP levels decrease and the activity of ATP-dependent ion pumps such as the Na+/K+-ATPase is slowed down, causing the membrane potential to shift toward hypopolarization. Neurotransmitters are released, and their uptake is delayed.	topic_bd
77660	10	356111	7	NULL	NULL	0	NULL	Na+/K+-ATPase	GP	activity of	slowed down					OXPHOS	Process	under compromised			NULL		0	NULL	NULL	NULL	NULL	NULL	Gene and protein expression profiles in BPD show a decrease of mRNA and proteins involved in mitochondrial functions such as oxidative phosphorylation (OXPHOS) (Iwamoto et al., 2005 K. Iwamoto, M. Bundo and T. Kato, Altered expression of mitochondria-related genes in postmortem brains of patients with bipolar disorder or schizophrenia, as revealed by large-scale DNA microarray analysis, Hum. Mol. Genet. 14 (2005), pp. 241–253. View Record in Scopus | Cited By in Scopus (130)[Iwamoto et al., 2005], [Konradi et al., 2004], [Pennington et al., 2008] and [Washizuka et al., 2005]). Downregulations were observed in the prefrontal cortex (PFC; Brodmann areas 9 and 46, Table 1), ([Iwamoto et al., 2005], [Pennington et al., 2008] and [Sun et al., 2006]), hippocampus (Konradi et al., 2004) and in lymphoblastoid cell lines (Table 2), (Washizuka et al., 2005). Under compromised OXPHOS, ATP levels decrease and the activity of ATP-dependent ion pumps such as the Na+/K+-ATPase is slowed down, causing the membrane potential to shift toward hypopolarization. Neurotransmitters are released, and their uptake is delayed.	topic_bd
77661	11	356111	7	NULL	NULL	0	NULL	membrane potential	Process		shift toward					hypopolarization	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Gene and protein expression profiles in BPD show a decrease of mRNA and proteins involved in mitochondrial functions such as oxidative phosphorylation (OXPHOS) (Iwamoto et al., 2005 K. Iwamoto, M. Bundo and T. Kato, Altered expression of mitochondria-related genes in postmortem brains of patients with bipolar disorder or schizophrenia, as revealed by large-scale DNA microarray analysis, Hum. Mol. Genet. 14 (2005), pp. 241–253. View Record in Scopus | Cited By in Scopus (130)[Iwamoto et al., 2005], [Konradi et al., 2004], [Pennington et al., 2008] and [Washizuka et al., 2005]). Downregulations were observed in the prefrontal cortex (PFC; Brodmann areas 9 and 46, Table 1), ([Iwamoto et al., 2005], [Pennington et al., 2008] and [Sun et al., 2006]), hippocampus (Konradi et al., 2004) and in lymphoblastoid cell lines (Table 2), (Washizuka et al., 2005). Under compromised OXPHOS, ATP levels decrease and the activity of ATP-dependent ion pumps such as the Na+/K+-ATPase is slowed down, causing the membrane potential to shift toward hypopolarization. Neurotransmitters are released, and their uptake is delayed.	topic_bd
77663	12	356111	7	NULL	NULL	NULL	NULL	statement 10	Process		cause					statement 11	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene and protein expression profiles in BPD show a decrease of mRNA and proteins involved in mitochondrial functions such as oxidative phosphorylation (OXPHOS) (Iwamoto et al., 2005 K. Iwamoto, M. Bundo and T. Kato, Altered expression of mitochondria-related genes in postmortem brains of patients with bipolar disorder or schizophrenia, as revealed by large-scale DNA microarray analysis, Hum. Mol. Genet. 14 (2005), pp. 241–253. View Record in Scopus | Cited By in Scopus (130)[Iwamoto et al., 2005], [Konradi et al., 2004], [Pennington et al., 2008] and [Washizuka et al., 2005]). Downregulations were observed in the prefrontal cortex (PFC; Brodmann areas 9 and 46, Table 1), ([Iwamoto et al., 2005], [Pennington et al., 2008] and [Sun et al., 2006]), hippocampus (Konradi et al., 2004) and in lymphoblastoid cell lines (Table 2), (Washizuka et al., 2005). Under compromised OXPHOS, ATP levels decrease and the activity of ATP-dependent ion pumps such as the Na+/K+-ATPase is slowed down, causing the membrane potential to shift toward hypopolarization. Neurotransmitters are released, and their uptake is delayed.	topic_bd
77664	13	356111	7	NULL	NULL	NULL	NULL	neurotransmitters	Chemical		are					released	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene and protein expression profiles in BPD show a decrease of mRNA and proteins involved in mitochondrial functions such as oxidative phosphorylation (OXPHOS) (Iwamoto et al., 2005 K. Iwamoto, M. Bundo and T. Kato, Altered expression of mitochondria-related genes in postmortem brains of patients with bipolar disorder or schizophrenia, as revealed by large-scale DNA microarray analysis, Hum. Mol. Genet. 14 (2005), pp. 241–253. View Record in Scopus | Cited By in Scopus (130)[Iwamoto et al., 2005], [Konradi et al., 2004], [Pennington et al., 2008] and [Washizuka et al., 2005]). Downregulations were observed in the prefrontal cortex (PFC; Brodmann areas 9 and 46, Table 1), ([Iwamoto et al., 2005], [Pennington et al., 2008] and [Sun et al., 2006]), hippocampus (Konradi et al., 2004) and in lymphoblastoid cell lines (Table 2), (Washizuka et al., 2005). Under compromised OXPHOS, ATP levels decrease and the activity of ATP-dependent ion pumps such as the Na+/K+-ATPase is slowed down, causing the membrane potential to shift toward hypopolarization. Neurotransmitters are released, and their uptake is delayed.	topic_bd
77665	14	356111	7	NULL	NULL	NULL	NULL	neurotransmitter	Chemical	uptake of	is					delayed	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene and protein expression profiles in BPD show a decrease of mRNA and proteins involved in mitochondrial functions such as oxidative phosphorylation (OXPHOS) (Iwamoto et al., 2005 K. Iwamoto, M. Bundo and T. Kato, Altered expression of mitochondria-related genes in postmortem brains of patients with bipolar disorder or schizophrenia, as revealed by large-scale DNA microarray analysis, Hum. Mol. Genet. 14 (2005), pp. 241–253. View Record in Scopus | Cited By in Scopus (130)[Iwamoto et al., 2005], [Konradi et al., 2004], [Pennington et al., 2008] and [Washizuka et al., 2005]). Downregulations were observed in the prefrontal cortex (PFC; Brodmann areas 9 and 46, Table 1), ([Iwamoto et al., 2005], [Pennington et al., 2008] and [Sun et al., 2006]), hippocampus (Konradi et al., 2004) and in lymphoblastoid cell lines (Table 2), (Washizuka et al., 2005). Under compromised OXPHOS, ATP levels decrease and the activity of ATP-dependent ion pumps such as the Na+/K+-ATPase is slowed down, causing the membrane potential to shift toward hypopolarization. Neurotransmitters are released, and their uptake is delayed.	topic_bd
77666	15	356111	7	NULL	NULL	0	NULL	statement 10	Process		cause					statement 14	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Gene and protein expression profiles in BPD show a decrease of mRNA and proteins involved in mitochondrial functions such as oxidative phosphorylation (OXPHOS) (Iwamoto et al., 2005 K. Iwamoto, M. Bundo and T. Kato, Altered expression of mitochondria-related genes in postmortem brains of patients with bipolar disorder or schizophrenia, as revealed by large-scale DNA microarray analysis, Hum. Mol. Genet. 14 (2005), pp. 241–253. View Record in Scopus | Cited By in Scopus (130)[Iwamoto et al., 2005], [Konradi et al., 2004], [Pennington et al., 2008] and [Washizuka et al., 2005]). Downregulations were observed in the prefrontal cortex (PFC; Brodmann areas 9 and 46, Table 1), ([Iwamoto et al., 2005], [Pennington et al., 2008] and [Sun et al., 2006]), hippocampus (Konradi et al., 2004) and in lymphoblastoid cell lines (Table 2), (Washizuka et al., 2005). Under compromised OXPHOS, ATP levels decrease and the activity of ATP-dependent ion pumps such as the Na+/K+-ATPase is slowed down, causing the membrane potential to shift toward hypopolarization. Neurotransmitters are released, and their uptake is delayed.	topic_bd
77667	1	356112	7	NULL	NULL	0	NULL	pH	QuantityOrMeasure	reduced frontal lobe	occur in					BPD patients	MedicalFinding	medicated			NULL		0	NULL	NULL	NULL	NULL	NULL	Kato et al. found reduced frontal lobe pH in medicated and unmedicated BPD patients ([Kato et al., 1998] and [Kato et al., 1993]), and two-dimensional proton echo-planar spectroscopic imaging of medication-free BPD patients showed a shift from OXPHOS to glycolysis (Dager et al., 2004 S.R. Dager et al., Brain metabolic alterations in medication-free patients with bipolar disorder, Arch. Gen. Psychiatry 61 (2004), pp. 450–458. Full Text via CrossRef | View Record in Scopus | Cited By in Scopus (137)Dager et al., 2004), (Fig. 1).	topic_bd
77668	2	356112	7	NULL	NULL	0	NULL	pH	QuantityOrMeasure	reduced frontal lobe	occur in					BPD patients	MedicalFinding	unmedicated			NULL		0	NULL	NULL	NULL	NULL	NULL	Kato et al. found reduced frontal lobe pH in medicated and unmedicated BPD patients ([Kato et al., 1998] and [Kato et al., 1993]), and two-dimensional proton echo-planar spectroscopic imaging of medication-free BPD patients showed a shift from OXPHOS to glycolysis (Dager et al., 2004 S.R. Dager et al., Brain metabolic alterations in medication-free patients with bipolar disorder, Arch. Gen. Psychiatry 61 (2004), pp. 450–458. Full Text via CrossRef | View Record in Scopus | Cited By in Scopus (137)Dager et al., 2004), (Fig. 1).	topic_bd
77669	3	356112	7	NULL	NULL	0	NULL	OXPHOS	Process		shifted to					glycolysis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Kato et al. found reduced frontal lobe pH in medicated and unmedicated BPD patients ([Kato et al., 1998] and [Kato et al., 1993]), and two-dimensional proton echo-planar spectroscopic imaging of medication-free BPD patients showed a shift from OXPHOS to glycolysis (Dager et al., 2004 S.R. Dager et al., Brain metabolic alterations in medication-free patients with bipolar disorder, Arch. Gen. Psychiatry 61 (2004), pp. 450–458. Full Text via CrossRef | View Record in Scopus | Cited By in Scopus (137)Dager et al., 2004), (Fig. 1).	topic_bd
77670	4	356112	7	NULL	NULL	0	NULL	statement 3	Process		occur in					BPD patients	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Kato et al. found reduced frontal lobe pH in medicated and unmedicated BPD patients ([Kato et al., 1998] and [Kato et al., 1993]), and two-dimensional proton echo-planar spectroscopic imaging of medication-free BPD patients showed a shift from OXPHOS to glycolysis (Dager et al., 2004 S.R. Dager et al., Brain metabolic alterations in medication-free patients with bipolar disorder, Arch. Gen. Psychiatry 61 (2004), pp. 450–458. Full Text via CrossRef | View Record in Scopus | Cited By in Scopus (137)Dager et al., 2004), (Fig. 1).	topic_bd
77671	1	356113	7	NULL	NULL	NULL	NULL	mRNA	NucleicAcid	lower levels of	occur in the					electron transfer chain	GP				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Specifically, lower mRNA and protein levels of the electron transfer chain cause a shift from OXPHOS to glycolysis to retain ATP production, which leads to the accumulation of lactic acid, the acidification of tissue, and a decrease in pH 	topic_bd
77672	2	356113	7	NULL	NULL	0	NULL	protein	GP	lower levels of	occur in the					electron transfer chain	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically, lower mRNA and protein levels of the electron transfer chain cause a shift from OXPHOS to glycolysis to retain ATP production, which leads to the accumulation of lactic acid, the acidification of tissue, and a decrease in pH 	topic_bd
77673	3	356113	7	NULL	NULL	0	NULL	OXPHOS	Process		shifted to					glycolysis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically, lower mRNA and protein levels of the electron transfer chain cause a shift from OXPHOS to glycolysis to retain ATP production, which leads to the accumulation of lactic acid, the acidification of tissue, and a decrease in pH 	topic_bd
77674	4	356113	7	NULL	NULL	0	NULL	statement 3	Process		retain					ATP	Chemical	production of			NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically, lower mRNA and protein levels of the electron transfer chain cause a shift from OXPHOS to glycolysis to retain ATP production, which leads to the accumulation of lactic acid, the acidification of tissue, and a decrease in pH 	topic_bd
77675	5	356113	7	NULL	NULL	0	NULL	statement 1	Process		cause					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically, lower mRNA and protein levels of the electron transfer chain cause a shift from OXPHOS to glycolysis to retain ATP production, which leads to the accumulation of lactic acid, the acidification of tissue, and a decrease in pH 	topic_bd
77676	6	356113	7	NULL	NULL	0	NULL	statement 2	Process		cause					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically, lower mRNA and protein levels of the electron transfer chain cause a shift from OXPHOS to glycolysis to retain ATP production, which leads to the accumulation of lactic acid, the acidification of tissue, and a decrease in pH 	topic_bd
77677	7	356113	7	NULL	NULL	0	NULL	statement 4	Process		leads to					lactic acid	Chemical	accumulation of			NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically, lower mRNA and protein levels of the electron transfer chain cause a shift from OXPHOS to glycolysis to retain ATP production, which leads to the accumulation of lactic acid, the acidification of tissue, and a decrease in pH 	topic_bd
77678	8	356113	7	NULL	NULL	0	NULL	statement 7	Process		leads to					tissue	OrganismPart	acidification of			NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically, lower mRNA and protein levels of the electron transfer chain cause a shift from OXPHOS to glycolysis to retain ATP production, which leads to the accumulation of lactic acid, the acidification of tissue, and a decrease in pH 	topic_bd
77679	9	356113	7	NULL	NULL	0	NULL	statement 8	Process		leads to					pH	QuantityOrMeasure	decrease of			NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically, lower mRNA and protein levels of the electron transfer chain cause a shift from OXPHOS to glycolysis to retain ATP production, which leads to the accumulation of lactic acid, the acidification of tissue, and a decrease in pH 	topic_bd
77382	1	356114	5	NULL	NULL	0	NULL	synaptic maturation	Process	delayed	is linked to					FXS	MedicalFinding	pathogenesis of			NULL		0	NULL	NULL	NULL	NULL	NULL	In particular, delayed synaptic maturation, abnormal synaptic structure and/or function and alterations in intracellular signaling pathways have been linked to the pathogenesis of FXS and ASD	topic_aut
77383	2	356114	5	NULL	NULL	0	NULL	synaptic maturation	Process	delayed	is linked to					ASD	MedicalFinding	pathogenesis of			NULL		0	NULL	NULL	NULL	NULL	NULL	In particular, delayed synaptic maturation, abnormal synaptic structure and/or function and alterations in intracellular signaling pathways have been linked to the pathogenesis of FXS and ASD	topic_aut
77384	3	356114	5	NULL	NULL	0	NULL	synapse	OrganismPart	abnormal;;structure of	is linked to					FXS	MedicalFinding	pathogenesis of			NULL		0	NULL	NULL	NULL	NULL	NULL	In particular, delayed synaptic maturation, abnormal synaptic structure and/or function and alterations in intracellular signaling pathways have been linked to the pathogenesis of FXS and ASD	topic_aut
77385	4	356114	5	NULL	NULL	0	NULL	synapse	OrganismPart	abnormal;;structure of	is linked to					ASD	MedicalFinding	pathogenesis of			NULL		0	NULL	NULL	NULL	NULL	NULL	In particular, delayed synaptic maturation, abnormal synaptic structure and/or function and alterations in intracellular signaling pathways have been linked to the pathogenesis of FXS and ASD	topic_aut
77386	5	356114	5	NULL	NULL	0	NULL	signaling pathways	Process	function of ;;intracellular	is linked to					FXS	MedicalFinding	pathogenesis of			NULL		0	NULL	NULL	NULL	NULL	NULL	In particular, delayed synaptic maturation, abnormal synaptic structure and/or function and alterations in intracellular signaling pathways have been linked to the pathogenesis of FXS and ASD	topic_aut
77387	6	356114	5	NULL	NULL	0	NULL	signaling pathways	Process	function of ;;intracellular	is linked to					ASD	MedicalFinding	pathogenesis of			NULL		0	NULL	NULL	NULL	NULL	NULL	In particular, delayed synaptic maturation, abnormal synaptic structure and/or function and alterations in intracellular signaling pathways have been linked to the pathogenesis of FXS and ASD	topic_aut
77388	7	356114	5	NULL	NULL	0	NULL	signaling pathways	Process	alterations of;;intracellular	is linked to					FXS	MedicalFinding	pathogenesis of			NULL		0	NULL	NULL	NULL	NULL	NULL	In particular, delayed synaptic maturation, abnormal synaptic structure and/or function and alterations in intracellular signaling pathways have been linked to the pathogenesis of FXS and ASD	topic_aut
77389	8	356114	5	NULL	NULL	0	NULL	signaling pathways	Process	alterations of;;intracellular	is linked to					ASD	MedicalFinding	pathogenesis of			NULL		0	NULL	NULL	NULL	NULL	NULL	In particular, delayed synaptic maturation, abnormal synaptic structure and/or function and alterations in intracellular signaling pathways have been linked to the pathogenesis of FXS and ASD	topic_aut
78064	1	356115	5	NULL	NULL	0	NULL	GABA(A) receptor	GP		is a type of					ion channel	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Aberrations in GABA(A) receptor ion channels and the G-protein coupled metabotropic glutamate and GABA(B) transmitter systems are also linked to both disorders and these receptors are currently at the forefront of preclinical and clinical research into treatments for both autism and Fragile X Syndrome.	topic_aut
78065	2	356115	5	NULL	NULL	0	NULL	GABA(A) receptor	GP	aberrations of	is linked to					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Aberrations in GABA(A) receptor ion channels and the G-protein coupled metabotropic glutamate and GABA(B) transmitter systems are also linked to both disorders and these receptors are currently at the forefront of preclinical and clinical research into treatments for both autism and Fragile X Syndrome.	topic_aut
78066	3	356115	5	NULL	NULL	0	NULL	GABA(A) receptor	GP	aberrations of	is linked to					Fragile X Syndrome	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Aberrations in GABA(A) receptor ion channels and the G-protein coupled metabotropic glutamate and GABA(B) transmitter systems are also linked to both disorders and these receptors are currently at the forefront of preclinical and clinical research into treatments for both autism and Fragile X Syndrome.	topic_aut
78071	4	356115	5	NULL	NULL	0	NULL	G-protein coupled metabotropic glutamate	GP	aberrations of	is linked to					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Aberrations in GABA(A) receptor ion channels and the G-protein coupled metabotropic glutamate and GABA(B) transmitter systems are also linked to both disorders and these receptors are currently at the forefront of preclinical and clinical research into treatments for both autism and Fragile X Syndrome.	topic_aut
78072	5	356115	5	NULL	NULL	0	NULL	G-protein coupled metabotropic glutamate	GP	aberrations of	is linked to					Fragile X Syndrome	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Aberrations in GABA(A) receptor ion channels and the G-protein coupled metabotropic glutamate and GABA(B) transmitter systems are also linked to both disorders and these receptors are currently at the forefront of preclinical and clinical research into treatments for both autism and Fragile X Syndrome.	topic_aut
78073	6	356115	5	NULL	NULL	0	NULL	G-protein coupled GABA(B) transmitter systems	GP	aberrations of	is linked to					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Aberrations in GABA(A) receptor ion channels and the G-protein coupled metabotropic glutamate and GABA(B) transmitter systems are also linked to both disorders and these receptors are currently at the forefront of preclinical and clinical research into treatments for both autism and Fragile X Syndrome.	topic_aut
78074	7	356115	5	NULL	NULL	0	NULL	G-protein coupled GABA(B) transmitter systems	GP	aberrations of	is linked to					Fragile X Syndrome	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Aberrations in GABA(A) receptor ion channels and the G-protein coupled metabotropic glutamate and GABA(B) transmitter systems are also linked to both disorders and these receptors are currently at the forefront of preclinical and clinical research into treatments for both autism and Fragile X Syndrome.	topic_aut
78075	1	356116	5	NULL	NULL	NULL	NULL	GAD1 gene	GP	common genetic variation of	unlikely to play a role in		critical			ASD	MedicalFinding	susceptibility of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our observations, when taken together with previous findings, suggest that common genetic variation in the GAD1 and DLX genes is unlikely to play a critical role in ASD susceptibility	topic_aut
78076	2	356116	5	NULL	NULL	0	NULL	DLX gene	GP	common genetic variation of	unlikely to play a role in		critical			ASD	MedicalFinding	susceptibility of			NULL		0	NULL	NULL	NULL	NULL	NULL	Our observations, when taken together with previous findings, suggest that common genetic variation in the GAD1 and DLX genes is unlikely to play a critical role in ASD susceptibility	topic_aut
78077	1	356117	5	NULL	NULL	0	NULL	GAD67	GP		is also known as					GAD1	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamate decarboxylase 1 (brain, 67kDa) (GAD67), also known as GAD1, is a human gene.[1] This gene encodes one of several forms of glutamic acid decarboxylase, identified as a major autoantigen in insulin-dependent diabetes	topic_aut
78078	2	356117	5	NULL	NULL	0	NULL	GAD67	GP		is					Glutamate decarboxylase 1 (brain, 67kDa) 	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamate decarboxylase 1 (brain, 67kDa) (GAD67), also known as GAD1, is a human gene.[1] This gene encodes one of several forms of glutamic acid decarboxylase, identified as a major autoantigen in insulin-dependent diabetes	topic_aut
78079	3	356117	5	NULL	NULL	0	NULL	GAD1	GP	human	encodes					glutamic acid decarboxylase	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamate decarboxylase 1 (brain, 67kDa) (GAD67), also known as GAD1, is a human gene.[1] This gene encodes one of several forms of glutamic acid decarboxylase, identified as a major autoantigen in insulin-dependent diabetes	topic_aut
78080	4	356117	5	NULL	NULL	0	NULL	glutamic acid decarboxylase	GP		is a type of					autoantigen	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamate decarboxylase 1 (brain, 67kDa) (GAD67), also known as GAD1, is a human gene.[1] This gene encodes one of several forms of glutamic acid decarboxylase, identified as a major autoantigen in insulin-dependent diabetes	topic_aut
78081	5	356117	5	NULL	NULL	0	NULL	statement 4	GP		is present in					 insulin-dependent diabetes	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamate decarboxylase 1 (brain, 67kDa) (GAD67), also known as GAD1, is a human gene.[1] This gene encodes one of several forms of glutamic acid decarboxylase, identified as a major autoantigen in insulin-dependent diabetes	topic_aut
78082	1	356118	5	NULL	NULL	0	NULL	Dlx	GP		is a family of					homeodomain transcription factors	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Dlx is a family of homeodomain transcription factors which are related to the Drosophila distal-less (Dll) gene [1]. The family has been related to a number of developmental features. The family seems to be well preserved across species[2].	topic_aut
78083	2	356118	5	NULL	NULL	0	NULL	Dlx	GP		is related to					Dll gene	GP	Drosophila			NULL		0	NULL	NULL	NULL	NULL	NULL	Dlx is a family of homeodomain transcription factors which are related to the Drosophila distal-less (Dll) gene [1]. The family has been related to a number of developmental features. The family seems to be well preserved across species[2].	topic_aut
78084	3	356118	5	NULL	NULL	0	NULL	Dll gene	GP		is					distal-less gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Dlx is a family of homeodomain transcription factors which are related to the Drosophila distal-less (Dll) gene [1]. The family has been related to a number of developmental features. The family seems to be well preserved across species[2].	topic_aut
78085	4	356118	5	NULL	NULL	0	NULL	Dlx	GP		is related to					developmental features	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Dlx is a family of homeodomain transcription factors which are related to the Drosophila distal-less (Dll) gene [1]. The family has been related to a number of developmental features. The family seems to be well preserved across species[2].	topic_aut
78115	1	356119	5	NULL	NULL	0	NULL	CNVs	NucleicAcid	rare	encompass					ASDs	MedicalFinding	potential;;candidate regions for			NULL		0	NULL	NULL	NULL	NULL	NULL	We conclude that rare CNVs, encompassing potential candidate regions for ASDs, increase the susceptibility for the development of ASDs and related neuropsychiatric disorders giving us further insight into the complex genetics underlying ASDs.	topic_aut
78116	2	356119	5	NULL	NULL	0	NULL	CNVs	NucleicAcid	rare	increases					ASDs	MedicalFinding	susceptibility of;;development of			NULL		0	NULL	NULL	NULL	NULL	NULL	We conclude that rare CNVs, encompassing potential candidate regions for ASDs, increase the susceptibility for the development of ASDs and related neuropsychiatric disorders giving us further insight into the complex genetics underlying ASDs.	topic_aut
78117	3	356119	5	NULL	NULL	0	NULL	CNVs	NucleicAcid	rare	increases					neuropsychiatric disorders	MedicalFinding	susceptibility of;;development of			NULL		0	NULL	NULL	NULL	NULL	NULL	We conclude that rare CNVs, encompassing potential candidate regions for ASDs, increase the susceptibility for the development of ASDs and related neuropsychiatric disorders giving us further insight into the complex genetics underlying ASDs.	topic_aut
78118	1	356120	5	NULL	NULL	0	NULL	SCARB2 gene	GP		is linked to					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The following candidate genes were identified in children with autism by in silico analysis: SCARB2, TPPP, PDCD6, SEPT5, GP1BB, PI4KA, NPTX1, STCH, NRIP1, and CXADR	topic_aut
78119	2	356120	5	NULL	NULL	0	NULL	TPPP gene	GP		is linked to					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The following candidate genes were identified in children with autism by in silico analysis: SCARB2, TPPP, PDCD6, SEPT5, GP1BB, PI4KA, NPTX1, STCH, NRIP1, and CXADR	topic_aut
78120	3	356120	5	NULL	NULL	0	NULL	PDCD6 gene	GP		is linked to					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The following candidate genes were identified in children with autism by in silico analysis: SCARB2, TPPP, PDCD6, SEPT5, GP1BB, PI4KA, NPTX1, STCH, NRIP1, and CXADR	topic_aut
78121	4	356120	5	NULL	NULL	0	NULL	SEPT5 gene	GP		is linked to					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The following candidate genes were identified in children with autism by in silico analysis: SCARB2, TPPP, PDCD6, SEPT5, GP1BB, PI4KA, NPTX1, STCH, NRIP1, and CXADR	topic_aut
78126	5	356120	5	NULL	NULL	0	NULL	GP1BB gene	GP		is linked to					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The following candidate genes were identified in children with autism by in silico analysis: SCARB2, TPPP, PDCD6, SEPT5, GP1BB, PI4KA, NPTX1, STCH, NRIP1, and CXADR	topic_aut
78128	6	356120	5	NULL	NULL	0	NULL	PI4KA gene	GP		is linked to					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The following candidate genes were identified in children with autism by in silico analysis: SCARB2, TPPP, PDCD6, SEPT5, GP1BB, PI4KA, NPTX1, STCH, NRIP1, and CXADR	topic_aut
78131	7	356120	5	NULL	NULL	0	NULL	NPTX1 gene	GP		is linked to					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The following candidate genes were identified in children with autism by in silico analysis: SCARB2, TPPP, PDCD6, SEPT5, GP1BB, PI4KA, NPTX1, STCH, NRIP1, and CXADR	topic_aut
78135	8	356120	5	NULL	NULL	0	NULL	STCH gene	GP		is linked to					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The following candidate genes were identified in children with autism by in silico analysis: SCARB2, TPPP, PDCD6, SEPT5, GP1BB, PI4KA, NPTX1, STCH, NRIP1, and CXADR	topic_aut
78136	9	356120	5	NULL	NULL	0	NULL	NRIP1 gene	GP		is linked to					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The following candidate genes were identified in children with autism by in silico analysis: SCARB2, TPPP, PDCD6, SEPT5, GP1BB, PI4KA, NPTX1, STCH, NRIP1, and CXADR	topic_aut
78138	10	356120	5	NULL	NULL	0	NULL	CXADR gene	GP		is linked to					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The following candidate genes were identified in children with autism by in silico analysis: SCARB2, TPPP, PDCD6, SEPT5, GP1BB, PI4KA, NPTX1, STCH, NRIP1, and CXADR	topic_aut
78139	1	356121	5	NULL	NULL	0	NULL	Lysosome membrane protein 2	GP	human	is encoded by					SCARB2 gene	GP	human			NULL		0	NULL	NULL	NULL	NULL	NULL	Lysosome membrane protein 2 is a protein that in humans is encoded by the SCARB2 gene	topic_aut
78141	1	356122	5	NULL	NULL	0	NULL	Tubulin polymerization-promoting protein	GP	human	is encoded by					TPPP gene	GP	human			NULL		0	NULL	NULL	NULL	NULL	NULL	Tubulin polymerization-promoting protein is a protein that in humans is encoded by the TPPP gene.	topic_aut
78143	1	356123	5	NULL	NULL	0	NULL	Programmed cell death protein 6	GP	human	is encoded by					PDCD6 gene	GP	human			NULL		0	NULL	NULL	NULL	NULL	NULL	Programmed cell death protein 6 is a protein that in humans is encoded by the PDCD6 gene	topic_aut
78149	1	356124	5	NULL	NULL	0	NULL	Septin-5 protein	GP	human	is encoded by					SEPT5 gene	GP	human			NULL		0	NULL	NULL	NULL	NULL	NULL	Septin-5 is a protein that in humans is encoded by the SEPT5 gene	topic_aut
78150	1	356126	5	NULL	NULL	0	NULL	Phosphatidylinositol 4-kinase alpha	GP	human	is a type of					enzyme	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphatidylinositol 4-kinase alpha is an enzyme that in humans is encoded by the PI4KA gene	topic_aut
78151	2	356126	5	NULL	NULL	0	NULL	Phosphatidylinositol 4-kinase alpha	GP	human	is encoded by					PI4KA gene	GP	human			NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphatidylinositol 4-kinase alpha is an enzyme that in humans is encoded by the PI4KA gene	topic_aut
78152	1	356127	5	NULL	NULL	0	NULL	NP1	GP		is					Neuronal pentraxin-1	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Neuronal pentraxin-1 (NP1) is a protein that in humans is encoded by the NPTX1 gene	topic_aut
78153	2	356127	5	NULL	NULL	0	NULL	NP1 protein	GP	human	is encoded by					NPTX1 gene	GP	human			NULL		0	NULL	NULL	NULL	NULL	NULL	Neuronal pentraxin-1 (NP1) is a protein that in humans is encoded by the NPTX1 gene	topic_aut
78154	1	356128	5	NULL	NULL	0	NULL	Heat shock 70 kDa protein 13	GP	human	is encoded by					HSPA13 gene	GP	human			NULL		0	NULL	NULL	NULL	NULL	NULL	Heat shock 70 kDa protein 13 is a protein that in humans is encoded by the HSPA13 gene.	topic_aut
78156	1	356129	5	NULL	NULL	0	NULL	Nuclear receptor-interacting protein 1	GP	human	is encoded by					NRIP1 gene	GP	human			NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear receptor-interacting protein 1 is a protein that in humans is encoded by the NRIP1 gene	topic_aut
78158	1	356130	5	NULL	NULL	0	NULL	CAR	GP		is					coxsackievirus and adenovirus receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Coxsackievirus and adenovirus receptor (CAR) is a protein that in humans is encoded by the CXADR gene	topic_aut
78159	2	356130	5	NULL	NULL	0	NULL	CAR gene	GP	human	is encoded by					CXADR gene	GP	human			NULL		0	NULL	NULL	NULL	NULL	NULL	Coxsackievirus and adenovirus receptor (CAR) is a protein that in humans is encoded by the CXADR gene	topic_aut
78166	1	356131	5	NULL	NULL	0	NULL	schizophrenia	MedicalFinding		is associated with					white matter	OrganismPart	widespread changes in;;structure of			NULL		0	NULL	NULL	NULL	NULL	NULL	Schizophrenia is associated with often widespread changes in white matter structure.	topic_sch
78242	1	356133	5	NULL	NULL	0	NULL	 frontostriatocingulate network	OrganismPart	decreased activation of	is associated with					decision making	MentalProcess	uncertinity of			NULL		0	NULL	NULL	NULL	NULL	NULL	Decision-making under uncertainty was associated with a significantly decreased activation in a frontostriatocingulate network in the schizophrenia group. Structurally, they exhibited increased radial diffusivity in temporal white matter that was negatively correlated with activation in parts of the frontostriatocingulate network.	topic_sch
78243	2	356133	5	NULL	NULL	0	NULL	statement 1	Process		occurs in					schizophrenia group	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Decision-making under uncertainty was associated with a significantly decreased activation in a frontostriatocingulate network in the schizophrenia group. Structurally, they exhibited increased radial diffusivity in temporal white matter that was negatively correlated with activation in parts of the frontostriatocingulate network.	topic_sch
78244	3	356133	5	NULL	NULL	0	NULL	radial diffusivity	AbstractConcept		is increased in					temporal white matter	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Decision-making under uncertainty was associated with a significantly decreased activation in a frontostriatocingulate network in the schizophrenia group. Structurally, they exhibited increased radial diffusivity in temporal white matter that was negatively correlated with activation in parts of the frontostriatocingulate network.	topic_sch
78245	4	356133	5	NULL	NULL	0	NULL	statement 3	Process		correlates with		negatively			frontostriatocingulate network	OrganismPart	activation of;;parts of			NULL		0	NULL	NULL	NULL	NULL	NULL	Decision-making under uncertainty was associated with a significantly decreased activation in a frontostriatocingulate network in the schizophrenia group. Structurally, they exhibited increased radial diffusivity in temporal white matter that was negatively correlated with activation in parts of the frontostriatocingulate network.	topic_sch
78246	1	356134	5	NULL	NULL	NULL	NULL	diffusivity	AbstractConcept		altered in					white matter networks	OrganismPart	relevant			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Present data indicate that altered diffusivity within relevant white matter networks may be closely linked to abnormal neural activation in schizophrenia.	topic_sch
78247	2	356134	5	NULL	NULL	0	NULL	statement 1	Process		is linked to		closely			neural activation	Process	abnormal			NULL		0	NULL	NULL	NULL	NULL	NULL	Present data indicate that altered diffusivity within relevant white matter networks may be closely linked to abnormal neural activation in schizophrenia.	topic_sch
78248	3	356134	5	NULL	NULL	0	NULL	statement 2	Process		occurs in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Present data indicate that altered diffusivity within relevant white matter networks may be closely linked to abnormal neural activation in schizophrenia.	topic_sch
77688	1	356135	7	NULL	NULL	NULL	NULL	bipolar disorder	MedicalFinding	patients with	impaired					social competence	MentalProcess				NULL		NULL	NULL	NULL	NULL	NULL	NULL	A subgroup of outpatients with bipolar disorder has impaired social competence, which, when present, worsened the impact of depression and cognitive impairment on social functioning.	topic_bd
77689	2	356135	7	NULL	NULL	0	NULL	statement 1	Process		worsens					depression	MedicalFinding	impact of			NULL		0	NULL	NULL	NULL	NULL	NULL	A subgroup of outpatients with bipolar disorder has impaired social competence, which, when present, worsened the impact of depression and cognitive impairment on social functioning.	topic_bd
77690	3	356135	7	NULL	NULL	0	NULL	statement 1	Process		worsens					social functioning	MentalProcess	cognitive impairment on			NULL		0	NULL	NULL	NULL	NULL	NULL	A subgroup of outpatients with bipolar disorder has impaired social competence, which, when present, worsened the impact of depression and cognitive impairment on social functioning.	topic_bd
77691	1	356136	7	NULL	NULL	0	NULL	Prodromal clinical phenomenology	MedicalProcedure		nonspecific to					FMAE	MedicalFinding	predict the occurrence of			NULL		0	NULL	NULL	NULL	NULL	NULL	Prodromal clinical phenomenology is too nonspecific to predict the occurrence of the FMAE of BD-II. However, identifiable subgroups may exist. We hypothesize that neurocognitive deficits together with pronounced irritability and aggressiveness may constitute a vulnerability marker for a subgroup of individuals who subsequently develop BD-II. This subgroup may be of potential interest for early identification.	topic_bd
77692	2	356136	7	NULL	NULL	0	NULL	statement 1	Process		occur in					BD-II	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Prodromal clinical phenomenology is too nonspecific to predict the occurrence of the FMAE of BD-II. However, identifiable subgroups may exist. We hypothesize that neurocognitive deficits together with pronounced irritability and aggressiveness may constitute a vulnerability marker for a subgroup of individuals who subsequently develop BD-II. This subgroup may be of potential interest for early identification.	topic_bd
77693	3	356136	7	NULL	NULL	0	NULL	neurocognitive deficits 	MedicalFinding		vulnerability marker for		may be			BD-II	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Prodromal clinical phenomenology is too nonspecific to predict the occurrence of the FMAE of BD-II. However, identifiable subgroups may exist. We hypothesize that neurocognitive deficits together with pronounced irritability and aggressiveness may constitute a vulnerability marker for a subgroup of individuals who subsequently develop BD-II. This subgroup may be of potential interest for early identification.	topic_bd
77694	4	356136	7	NULL	NULL	0	NULL	statement 3	Process		occur with					irritability	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Prodromal clinical phenomenology is too nonspecific to predict the occurrence of the FMAE of BD-II. However, identifiable subgroups may exist. We hypothesize that neurocognitive deficits together with pronounced irritability and aggressiveness may constitute a vulnerability marker for a subgroup of individuals who subsequently develop BD-II. This subgroup may be of potential interest for early identification.	topic_bd
77695	5	356136	7	NULL	NULL	0	NULL	statement 3	Process		occur with					aggressiveness	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Prodromal clinical phenomenology is too nonspecific to predict the occurrence of the FMAE of BD-II. However, identifiable subgroups may exist. We hypothesize that neurocognitive deficits together with pronounced irritability and aggressiveness may constitute a vulnerability marker for a subgroup of individuals who subsequently develop BD-II. This subgroup may be of potential interest for early identification.	topic_bd
78249	1	356137	5	NULL	NULL	0	NULL	autistic people	GroupOfPeople		cannot eaisly recognize					faces	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Researchers have long known, for example, that people with autism have difficulty recognizing faces.	topic_aut
78250	1	356138	5	NULL	NULL	0	NULL	people	GroupOfPeople		recognize		better			right-side up faces	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	While most people are better at recognizing images of faces when they are right-side up, autistic subjects identify them faster when they are upside-down	topic_aut
78251	2	356138	5	NULL	NULL	0	NULL	autistic subjects	GroupOfPeople		identify		faster			upsie-down faces	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	While most people are better at recognizing images of faces when they are right-side up, autistic subjects identify them faster when they are upside-down	topic_aut
78252	1	356139	5	NULL	NULL	0	NULL	brain area	OrganismPart		is involved with					object recognition	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	when autistic adolescents and adults were shown pictures of faces, another brain area involved with object recognition was activated, while the fusiform gyrus remained quiet.	topic_aut
78253	2	356139	5	NULL	NULL	0	NULL	statement 1	Process		is activated in					autistic adolescents	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	when autistic adolescents and adults were shown pictures of faces, another brain area involved with object recognition was activated, while the fusiform gyrus remained quiet.	topic_aut
78254	3	356139	5	NULL	NULL	0	NULL	faces	OrganismPart	seeing	leads to					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	when autistic adolescents and adults were shown pictures of faces, another brain area involved with object recognition was activated, while the fusiform gyrus remained quiet.	topic_aut
78255	4	356139	5	NULL	NULL	0	NULL	statement 1	Process		is activated in					autistic adults	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	when autistic adolescents and adults were shown pictures of faces, another brain area involved with object recognition was activated, while the fusiform gyrus remained quiet.	topic_aut
78256	5	356139	5	NULL	NULL	0	NULL	faces	OrganismPart	seeing	leads to					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	when autistic adolescents and adults were shown pictures of faces, another brain area involved with object recognition was activated, while the fusiform gyrus remained quiet.	topic_aut
78257	6	356139	5	NULL	NULL	0	NULL	fusiform gyrus	OrganismPart		is not active in					autistic adolescents	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	when autistic adolescents and adults were shown pictures of faces, another brain area involved with object recognition was activated, while the fusiform gyrus remained quiet.	topic_aut
78258	7	356139	5	NULL	NULL	0	NULL	fusiform gyrus	OrganismPart		is not active in					autistic adults	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	when autistic adolescents and adults were shown pictures of faces, another brain area involved with object recognition was activated, while the fusiform gyrus remained quiet.	topic_aut
78259	8	356139	5	NULL	NULL	0	NULL	faces	OrganismPart	seeing	leads to					statement 6	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	when autistic adolescents and adults were shown pictures of faces, another brain area involved with object recognition was activated, while the fusiform gyrus remained quiet.	topic_aut
78260	9	356139	5	NULL	NULL	0	NULL	faces	OrganismPart		leads to					statement 7	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	when autistic adolescents and adults were shown pictures of faces, another brain area involved with object recognition was activated, while the fusiform gyrus remained quiet.	topic_aut
78261	1	356140	5	NULL	NULL	0	NULL	fusiform gyrus	OrganismPart		is a component of					social brain	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	the fusiform gyrus may be a component of the social brain, intimately tied up with basic emotional responses like fear, anxiety and love.	topic_aut
78262	2	356140	5	NULL	NULL	0	NULL	fusiform gyrus	OrganismPart		is tied up with		intimately			fear	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	the fusiform gyrus may be a component of the social brain, intimately tied up with basic emotional responses like fear, anxiety and love.	topic_aut
78263	3	356140	5	NULL	NULL	0	NULL	fusiform gyrus	OrganismPart		is tied up with		intimately			anxiety	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	the fusiform gyrus may be a component of the social brain, intimately tied up with basic emotional responses like fear, anxiety and love.	topic_aut
78264	4	356140	5	NULL	NULL	0	NULL	fusiform gyrus	OrganismPart		is tied up with		intimately			love	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	the fusiform gyrus may be a component of the social brain, intimately tied up with basic emotional responses like fear, anxiety and love.	topic_aut
78265	5	356140	5	NULL	NULL	0	NULL	fear	MentalProcess		is a type of					emotional response	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	the fusiform gyrus may be a component of the social brain, intimately tied up with basic emotional responses like fear, anxiety and love.	topic_aut
78266	6	356140	5	NULL	NULL	0	NULL	anxiety	MentalProcess		is a type of					emotional response	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	the fusiform gyrus may be a component of the social brain, intimately tied up with basic emotional responses like fear, anxiety and love.	topic_aut
78267	7	356140	5	NULL	NULL	0	NULL	love	MentalProcess		is a type of					emotional response	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	the fusiform gyrus may be a component of the social brain, intimately tied up with basic emotional responses like fear, anxiety and love.	topic_aut
78648	1	356141	5	NULL	NULL	0	NULL	neurons	Cell	stacks of	is known as					mini-columns	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	an increase in autistic brains in the stacks of neurons known as mini-columns that extend through the layers of the neocortex. The brains of people with autism not only had more mini-columns, Dr. Casanova found, but the neurons that made up the columns were less variable in size than in normal brains	topic_aut
78649	2	356141	5	NULL	NULL	NULL	NULL	mini-columns	OrganismPart		extend through					neocortex	OrganismPart	layers of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	an increase in autistic brains in the stacks of neurons known as mini-columns that extend through the layers of the neocortex. The brains of people with autism not only had more mini-columns, Dr. Casanova found, but the neurons that made up the columns were less variable in size than in normal brains	topic_aut
78650	3	356141	5	NULL	NULL	0	NULL	mini-columns	OrganismPart	more	is present in					autistic people	GroupOfPeople	brains of			NULL		0	NULL	NULL	NULL	NULL	NULL	an increase in autistic brains in the stacks of neurons known as mini-columns that extend through the layers of the neocortex. The brains of people with autism not only had more mini-columns, Dr. Casanova found, but the neurons that made up the columns were less variable in size than in normal brains	topic_aut
78651	4	356141	5	NULL	NULL	0	NULL	neurons	Cell	size of	is variable in					brain	OrganismPart	autistic			NULL		0	NULL	NULL	NULL	NULL	NULL	an increase in autistic brains in the stacks of neurons known as mini-columns that extend through the layers of the neocortex. The brains of people with autism not only had more mini-columns, Dr. Casanova found, but the neurons that made up the columns were less variable in size than in normal brains	topic_aut
78652	5	356141	5	NULL	NULL	0	NULL	neurons	Cell	size of	is variable in					brain	OrganismPart	normal			NULL		0	NULL	NULL	NULL	NULL	NULL	an increase in autistic brains in the stacks of neurons known as mini-columns that extend through the layers of the neocortex. The brains of people with autism not only had more mini-columns, Dr. Casanova found, but the neurons that made up the columns were less variable in size than in normal brains	topic_aut
78653	6	356141	5	NULL	NULL	0	NULL	statement 4	Process		lesser than					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	an increase in autistic brains in the stacks of neurons known as mini-columns that extend through the layers of the neocortex. The brains of people with autism not only had more mini-columns, Dr. Casanova found, but the neurons that made up the columns were less variable in size than in normal brains	topic_aut
78268	1	356142	5	NULL	NULL	0	NULL	mini-columns	OrganismPart	proliferation of	results in		might			stimulation	Process	deluge of			NULL		0	NULL	NULL	NULL	NULL	NULL	Dr. Casanova, for his part, theorizes that the proliferation of mini-columns might result in a deluge of stimulation, or as he puts it, ''way too much information.'	topic_aut
78269	1	356143	5	NULL	NULL	0	NULL	infants	GroupOfPeople	male	is genetically vulnerable to					stresses	PhysicalPhenomenon	early			NULL		0	NULL	NULL	NULL	NULL	NULL	We postulate that higher TST levels and, therefore, higher amounts of arousal-related inputs to the amygdala sensitize these genetically vulnerable male infants to very early stresses	topic_aut
78270	2	356143	5	NULL	NULL	0	NULL	TST	GP	higher levels of	leads to					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	We postulate that higher TST levels and, therefore, higher amounts of arousal-related inputs to the amygdala sensitize these genetically vulnerable male infants to very early stresses	topic_aut
78271	3	356143	5	NULL	NULL	0	NULL	TST	GP	higher levels of	leads to					arousal-related inputs	AbstractConcept	higher amounts of			NULL	amygdala	0	NULL	NULL	NULL	NULL	NULL	We postulate that higher TST levels and, therefore, higher amounts of arousal-related inputs to the amygdala sensitize these genetically vulnerable male infants to very early stresses	topic_aut
78272	4	356143	5	NULL	NULL	0	NULL	statement 3	Process		leads to					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	We postulate that higher TST levels and, therefore, higher amounts of arousal-related inputs to the amygdala sensitize these genetically vulnerable male infants to very early stresses	topic_aut
78273	1	356145	5	NULL	NULL	0	NULL	oxidative stress	PhysicalPhenomenon		is implicated in					autism	MedicalFinding	pathophysiology of			NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidative stress and abnormal DNA methylation have been implicated in the pathophysiology of autism	topic_aut
78274	2	356145	5	NULL	NULL	0	NULL	DNA	NucleicAcid	abnormal methylation of	is implicated in					autism	MedicalFinding	pathophysiology of			NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidative stress and abnormal DNA methylation have been implicated in the pathophysiology of autism	topic_aut
78275	1	356146	5	NULL	NULL	0	NULL	antioxidant	Chemical	deficit in	is specific for					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that the deficit in antioxidant and methylation capacity is specific for autism and may promote cellular damage and altered epigenetic gene expression	topic_aut
78276	2	356146	5	NULL	NULL	0	NULL	antioxidant	Chemical	deficit in	promote		may			cellular damage	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that the deficit in antioxidant and methylation capacity is specific for autism and may promote cellular damage and altered epigenetic gene expression	topic_aut
78277	3	356146	5	NULL	NULL	NULL	NULL	antioxidant	Chemical	deficit in	promote		may			gene expression	Process	altered;;epigenetic			NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data indicate that the deficit in antioxidant and methylation capacity is specific for autism and may promote cellular damage and altered epigenetic gene expression	topic_aut
78278	4	356146	5	NULL	NULL	0	NULL	methylation capacity	Process		is specific for					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that the deficit in antioxidant and methylation capacity is specific for autism and may promote cellular damage and altered epigenetic gene expression	topic_aut
78290	1	356147	5	NULL	NULL	NULL	NULL	communication	MentalProcess	problems of	is a symptom of		prevalent			ASDs	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Communication problems and language delay are a prevalent symptom of autism spectrum disorders (ASDs)	topic_aut
78291	2	356147	5	NULL	NULL	0	NULL	language	MentalProcess	delay of	is a symptom of		prevalent			ASDs	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Communication problems and language delay are a prevalent symptom of autism spectrum disorders (ASDs)	topic_aut
78292	3	356147	5	NULL	NULL	0	NULL	ASDs	MedicalFinding		is					autism spectrum disorders	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Communication problems and language delay are a prevalent symptom of autism spectrum disorders (ASDs)	topic_aut
78293	1	356148	5	NULL	NULL	0	NULL	language	MentalProcess	delay of	is a symptom of					ASD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We detected candidate single-nucleotide polymorphisms (SNPs) in chromosome 11, rs11212733 (p-value=9.76×10(-6)) and rs7125479 (p-value=1.48×10(-4)), as a marker of language delay in ASD using the transmission disequilibrium test and multifactor dimensionality reduction test	topic_aut
78294	2	356148	5	NULL	NULL	0	NULL	SNPs	NucleicAcid		is					single-nucleotide polymorphisms	NucleicAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	We detected candidate single-nucleotide polymorphisms (SNPs) in chromosome 11, rs11212733 (p-value=9.76×10(-6)) and rs7125479 (p-value=1.48×10(-4)), as a marker of language delay in ASD using the transmission disequilibrium test and multifactor dimensionality reduction test	topic_aut
78295	3	356148	5	NULL	NULL	0	NULL	rs11212733	NucleicAcid		is a type of					SNPs	NucleicAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	We detected candidate single-nucleotide polymorphisms (SNPs) in chromosome 11, rs11212733 (p-value=9.76×10(-6)) and rs7125479 (p-value=1.48×10(-4)), as a marker of language delay in ASD using the transmission disequilibrium test and multifactor dimensionality reduction test	topic_aut
78296	4	356148	5	NULL	NULL	0	NULL	rs11212733	NucleicAcid		is present in					chromosome 11	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	We detected candidate single-nucleotide polymorphisms (SNPs) in chromosome 11, rs11212733 (p-value=9.76×10(-6)) and rs7125479 (p-value=1.48×10(-4)), as a marker of language delay in ASD using the transmission disequilibrium test and multifactor dimensionality reduction test	topic_aut
78297	5	356148	5	NULL	NULL	0	NULL	rs11212733	NucleicAcid		is a marker of					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	We detected candidate single-nucleotide polymorphisms (SNPs) in chromosome 11, rs11212733 (p-value=9.76×10(-6)) and rs7125479 (p-value=1.48×10(-4)), as a marker of language delay in ASD using the transmission disequilibrium test and multifactor dimensionality reduction test	topic_aut
78298	6	356148	5	NULL	NULL	0	NULL	rs7125479	NucleicAcid		is a type of					SNPs	NucleicAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	We detected candidate single-nucleotide polymorphisms (SNPs) in chromosome 11, rs11212733 (p-value=9.76×10(-6)) and rs7125479 (p-value=1.48×10(-4)), as a marker of language delay in ASD using the transmission disequilibrium test and multifactor dimensionality reduction test	topic_aut
78299	7	356148	5	NULL	NULL	0	NULL	rs7125479	NucleicAcid		is present in					chromosome 11	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	We detected candidate single-nucleotide polymorphisms (SNPs) in chromosome 11, rs11212733 (p-value=9.76×10(-6)) and rs7125479 (p-value=1.48×10(-4)), as a marker of language delay in ASD using the transmission disequilibrium test and multifactor dimensionality reduction test	topic_aut
78300	8	356148	5	NULL	NULL	0	NULL	rs7125479	NucleicAcid		is a marker of					ASD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We detected candidate single-nucleotide polymorphisms (SNPs) in chromosome 11, rs11212733 (p-value=9.76×10(-6)) and rs7125479 (p-value=1.48×10(-4)), as a marker of language delay in ASD using the transmission disequilibrium test and multifactor dimensionality reduction test	topic_aut
78301	1	356149	5	NULL	NULL	0	NULL	Melatonin	GP	administration of	is associated with					sleep	Process	improved parameters of			NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin administration in ASD is associated with improved sleep parameters, better daytime behavior, and minimal side effects	topic_aut
78302	2	356149	5	NULL	NULL	0	NULL	statement 1	Process		occurs in					ASD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin administration in ASD is associated with improved sleep parameters, better daytime behavior, and minimal side effects	topic_aut
78303	3	356149	5	NULL	NULL	0	NULL	Melatonin	GP	administration of	is associated with					daytime behavior	MentalProcess	better			NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin administration in ASD is associated with improved sleep parameters, better daytime behavior, and minimal side effects	topic_aut
78304	4	356149	5	NULL	NULL	0	NULL	statement 3	Process		occurs in					ASD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin administration in ASD is associated with improved sleep parameters, better daytime behavior, and minimal side effects	topic_aut
78305	5	356149	5	NULL	NULL	0	NULL	Melatonin	GP	administration of	is associated with					side effects	AbstractConcept	minimal			NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin administration in ASD is associated with improved sleep parameters, better daytime behavior, and minimal side effects	topic_aut
78306	6	356149	5	NULL	NULL	0	NULL	statement 5	Process		occurs in					ASD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin administration in ASD is associated with improved sleep parameters, better daytime behavior, and minimal side effects	topic_aut
78307	1	356150	5	NULL	NULL	0	NULL	SNAP-25 gene	GP		is involved in					neurotransmission	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The finding that polymorphisms of the SNAP-25 gene, a gene involved in neurotransmission and regulation of calcium homeostasis, are associated with the degree of hyperactivity in children with ASD, reinforces the hypothesis that alterations of these mechanisms play a pivotal role in the events leading to ASD-associated behavioral impairment	topic_aut
78308	2	356150	5	NULL	NULL	0	NULL	SNAP-25 gene	GP		regulates					calcium homeostasis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The finding that polymorphisms of the SNAP-25 gene, a gene involved in neurotransmission and regulation of calcium homeostasis, are associated with the degree of hyperactivity in children with ASD, reinforces the hypothesis that alterations of these mechanisms play a pivotal role in the events leading to ASD-associated behavioral impairment	topic_aut
78309	3	356150	5	NULL	NULL	0	NULL	hyperactivity	MedicalFinding		is a symptom of					ASD children	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	The finding that polymorphisms of the SNAP-25 gene, a gene involved in neurotransmission and regulation of calcium homeostasis, are associated with the degree of hyperactivity in children with ASD, reinforces the hypothesis that alterations of these mechanisms play a pivotal role in the events leading to ASD-associated behavioral impairment	topic_aut
78310	4	356150	5	NULL	NULL	0	NULL	SNAP-25 gene	GP	polymorphism of	is associated with					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The finding that polymorphisms of the SNAP-25 gene, a gene involved in neurotransmission and regulation of calcium homeostasis, are associated with the degree of hyperactivity in children with ASD, reinforces the hypothesis that alterations of these mechanisms play a pivotal role in the events leading to ASD-associated behavioral impairment	topic_aut
78311	1	356151	5	NULL	NULL	0	NULL	GLOI	GP		is					glyoxalase I gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	We have shown that a non-conservative, non-synonymous SNP in the glyoxalase I gene, GLOI, may be an autism susceptibility factor. The GLOI rs2736654 SNP is a C→A change that causes an Ala111Glu change in the Glo1 enzyme.	topic_aut
78312	2	356151	5	NULL	NULL	NULL	NULL	SNP	NucleicAcid	non-conservative;;non-synonymous	occurs in					GLOI	GP				NULL		NULL	NULL	NULL	NULL	NULL	NULL	We have shown that a non-conservative, non-synonymous SNP in the glyoxalase I gene, GLOI, may be an autism susceptibility factor. The GLOI rs2736654 SNP is a C→A change that causes an Ala111Glu change in the Glo1 enzyme.	topic_aut
78313	3	356151	5	NULL	NULL	0	NULL	statement 2	Process		is a type of					autism susceptibility factor	NucleicAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	We have shown that a non-conservative, non-synonymous SNP in the glyoxalase I gene, GLOI, may be an autism susceptibility factor. The GLOI rs2736654 SNP is a C→A change that causes an Ala111Glu change in the Glo1 enzyme.	topic_aut
78314	4	356151	5	NULL	NULL	0	NULL	GLOI rs2736654 SNP	NucleicAcid		is					C??A change	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	We have shown that a non-conservative, non-synonymous SNP in the glyoxalase I gene, GLOI, may be an autism susceptibility factor. The GLOI rs2736654 SNP is a C→A change that causes an Ala111Glu change in the Glo1 enzyme.	topic_aut
78315	5	356151	5	NULL	NULL	0	NULL	statement 4	Process		causes					Ala111Glu change	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	We have shown that a non-conservative, non-synonymous SNP in the glyoxalase I gene, GLOI, may be an autism susceptibility factor. The GLOI rs2736654 SNP is a C→A change that causes an Ala111Glu change in the Glo1 enzyme.	topic_aut
78316	6	356151	5	NULL	NULL	0	NULL	statement 5	Process		occurs in					Glo1 enzyme	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	We have shown that a non-conservative, non-synonymous SNP in the glyoxalase I gene, GLOI, may be an autism susceptibility factor. The GLOI rs2736654 SNP is a C→A change that causes an Ala111Glu change in the Glo1 enzyme.	topic_aut
77696	1	356154	7	NULL	NULL	0	NULL	childhood abuse	MentalProcess		is linked to					psychosis	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	A high prevalence of childhood abuse has been reported in patients with severe mental illness. We conducted a cross-sectional study of 102 patients with schizophrenia, bipolar disorder, or schizoaffective disorder. Social, demographic, and clinical data were obtained. Patients were evaluated using Brief Psychotic Relative Scale, and Traumatic Life Events and Distressing Event questionnaires. Almost half (47.5%) of these patients had suffered some kind of child abuse, and our results confirmed a relationship between a history of childhood abuse and more severe psychosis. Diagnosis of schizophrenia was determined 4.1 years earlier in victims of childhood abuse. Hospital admissions were twice as high in victims of psychological abuse. Patients with a history of sexual abuse were more than twice as likely to attempt suicide (68% vs. 28.9%).	topic_bd
77697	2	356154	7	NULL	NULL	0	NULL	childhood abuse	MentalProcess		reported in					mental illness	MedicalFinding	patients with			NULL		0	NULL	NULL	NULL	NULL	NULL	A high prevalence of childhood abuse has been reported in patients with severe mental illness. We conducted a cross-sectional study of 102 patients with schizophrenia, bipolar disorder, or schizoaffective disorder. Social, demographic, and clinical data were obtained. Patients were evaluated using Brief Psychotic Relative Scale, and Traumatic Life Events and Distressing Event questionnaires. Almost half (47.5%) of these patients had suffered some kind of child abuse, and our results confirmed a relationship between a history of childhood abuse and more severe psychosis. Diagnosis of schizophrenia was determined 4.1 years earlier in victims of childhood abuse. Hospital admissions were twice as high in victims of psychological abuse. Patients with a history of sexual abuse were more than twice as likely to attempt suicide (68% vs. 28.9%).	topic_bd
77698	1	356155	7	NULL	NULL	NULL	NULL	sexual abuse	MentalProcess	patients with history of	more likely to					suicide	MentalProcess	attempt			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patients with a history of sexual abuse were more than twice as likely to attempt suicide (68% vs. 28.9%).	topic_bd
77699	1	356156	7	NULL	NULL	NULL	NULL	GDs	MedicalFinding		found in					bipolar disorder	MedicalFinding	patients with			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Grandiose delusions (GDs) are found across a wide range of psychiatric conditions, including in around two-thirds of patients diagnosed with bipolar disorder, half of patients diagnosed with schizophrenia, as well as in a substantial proportion of patients with substance abuse disorders.	topic_bd
77700	2	356156	7	NULL	NULL	NULL	NULL	GDs	MedicalFinding		found in					schizophrenia	MedicalFinding	patients with			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Grandiose delusions (GDs) are found across a wide range of psychiatric conditions, including in around two-thirds of patients diagnosed with bipolar disorder, half of patients diagnosed with schizophrenia, as well as in a substantial proportion of patients with substance abuse disorders.	topic_bd
77701	3	356156	7	NULL	NULL	NULL	NULL	GDs	MedicalFinding		found in					substance abuse disorders	MedicalFinding	patients with			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Grandiose delusions (GDs) are found across a wide range of psychiatric conditions, including in around two-thirds of patients diagnosed with bipolar disorder, half of patients diagnosed with schizophrenia, as well as in a substantial proportion of patients with substance abuse disorders.	topic_bd
77702	4	356156	7	NULL	NULL	0	NULL	GDs	MedicalFinding		is					Grandiose delusions	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Grandiose delusions (GDs) are found across a wide range of psychiatric conditions, including in around two-thirds of patients diagnosed with bipolar disorder, half of patients diagnosed with schizophrenia, as well as in a substantial proportion of patients with substance abuse disorders.	topic_bd
77703	1	356157	7	NULL	NULL	0	NULL	mood symptoms	MentalProcess		associated with					 self-perceived stigma	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Objective The aim of this study was to investigate the impact of self-rated stigma and functioning in patients with previous termbipolar disordernext term in Latin-America. Methods Two-hundred and forty-one participants with previous termbipolar disordernext term were recruited from three Latin American countries (Argentina, Brazil, and Colombia). Functional impairment was assessed with the Functioning Assessment Short Test (FAST) and experiences with and impact of perceived stigma was evaluated using the Inventory of Stigmatizing Experiences (ISE). Results Higher scores of self-perceived stigma were correlated with lower scores of functioning. After multiple regression analysis, being on disability benefit, current mood symptoms and functioning were associated with self-perceived stigma. Conclusions This is the first study to demonstrate an association between stigma and poor functioning in previous termbipolar disorder.next term Possible implications of such findings for practitioners are discussed.	topic_bd
77704	2	356157	7	NULL	NULL	0	NULL	 self-perceived stigma	MentalProcess		associated with					previous termbipolar disorder	MedicalFinding	poor functioning in 			NULL		0	NULL	NULL	NULL	NULL	NULL	Objective The aim of this study was to investigate the impact of self-rated stigma and functioning in patients with previous termbipolar disordernext term in Latin-America. Methods Two-hundred and forty-one participants with previous termbipolar disordernext term were recruited from three Latin American countries (Argentina, Brazil, and Colombia). Functional impairment was assessed with the Functioning Assessment Short Test (FAST) and experiences with and impact of perceived stigma was evaluated using the Inventory of Stigmatizing Experiences (ISE). Results Higher scores of self-perceived stigma were correlated with lower scores of functioning. After multiple regression analysis, being on disability benefit, current mood symptoms and functioning were associated with self-perceived stigma. Conclusions This is the first study to demonstrate an association between stigma and poor functioning in previous termbipolar disorder.next term Possible implications of such findings for practitioners are discussed.	topic_bd
78070	1	356161	6	NULL	NULL	0	NULL	antimitotic drugs	Chemical		kill		may			tumor cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	How do antimitotic drugs kill cells in tumors? Timothy J. Mitchison, Harvard Medical School	topic_bc
78068	1	356164	6	NULL	NULL	0	NULL	metformin	Chemical		kills		selectively			cancer cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	an epigenetic switch linking inflammation to cancer and selective killing of cancer stem cells by metformin kevin struhl, harvard medical school	topic_bc
78069	2	356164	6	NULL	NULL	0	NULL	inflammation	MedicalFinding		is linked to					cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	an epigenetic switch linking inflammation to cancer and selective killing of cancer stem cells by metformin kevin struhl, harvard medical school	topic_bc
78067	1	356167	6	NULL	NULL	0	NULL	 jorge s reis-filno	MedicalFinding		is a type of					Breast cancer	MedicalFinding	metastatic			NULL		0	NULL	NULL	NULL	NULL	NULL	the molecular pathology of metaplastic breast cancer jorge s reis-filno	topic_bc
77705	1	356169	7	NULL	NULL	0	NULL	ECT	MedicalProcedure		is used in the					psychiatric disorders	MedicalFinding	somatic treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	Until recently, a review of nonpharmacological, somatic treatments of psychiatric disorders would have included only electroconvulsive therapy (ECT). This situation is now changing very substantially. Although ECT remains the only modality in widespread clinical use, several new techniques are under investigation. Their principal indication in the psychiatric context is the treatment of major depression, but other applications are also being studied. All the novel treatments involve brain stimulation, which is achieved by different technological methods. The treatment closest to the threshold of clinical acceptability is transcranial magnetic stimulation (TMS). Although TMS is safe and relatively easy to administer, its efficacy has still to be definitively established. Other modalities, at various stages of research development, include magnetic seizure therapy (MST), deep brain stimulation (DBS), and vagus nerve stimulation (VNS). We briefly review the development and technical aspects of these treatments, their potential role in the treatment of major depression, adverse effects, and putative mechanism of action. As the only one of these treatment modalities that is in widespread clinical use, more extended consideration is given to ECT Although more than half a century has elapsed since ECT was first introduced, it remains the most effective treatment for major depression, with efficacy in patients refractory to antidepressant drugs and an acceptable safety profile. Although they hold considerable promise, the novel brain stimulation techniques reviewed here will be need to be further developed before they achieve clinical acceptability.	topic_bd
77706	2	356169	7	NULL	NULL	0	NULL	ECT	MedicalProcedure		is					electroconvulsive therapy	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Until recently, a review of nonpharmacological, somatic treatments of psychiatric disorders would have included only electroconvulsive therapy (ECT). This situation is now changing very substantially. Although ECT remains the only modality in widespread clinical use, several new techniques are under investigation. Their principal indication in the psychiatric context is the treatment of major depression, but other applications are also being studied. All the novel treatments involve brain stimulation, which is achieved by different technological methods. The treatment closest to the threshold of clinical acceptability is transcranial magnetic stimulation (TMS). Although TMS is safe and relatively easy to administer, its efficacy has still to be definitively established. Other modalities, at various stages of research development, include magnetic seizure therapy (MST), deep brain stimulation (DBS), and vagus nerve stimulation (VNS). We briefly review the development and technical aspects of these treatments, their potential role in the treatment of major depression, adverse effects, and putative mechanism of action. As the only one of these treatment modalities that is in widespread clinical use, more extended consideration is given to ECT Although more than half a century has elapsed since ECT was first introduced, it remains the most effective treatment for major depression, with efficacy in patients refractory to antidepressant drugs and an acceptable safety profile. Although they hold considerable promise, the novel brain stimulation techniques reviewed here will be need to be further developed before they achieve clinical acceptability.	topic_bd
77707	3	356169	7	NULL	NULL	0	NULL	TMS	MedicalProcedure		is used in the					major depression	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	Until recently, a review of nonpharmacological, somatic treatments of psychiatric disorders would have included only electroconvulsive therapy (ECT). This situation is now changing very substantially. Although ECT remains the only modality in widespread clinical use, several new techniques are under investigation. Their principal indication in the psychiatric context is the treatment of major depression, but other applications are also being studied. All the novel treatments involve brain stimulation, which is achieved by different technological methods. The treatment closest to the threshold of clinical acceptability is transcranial magnetic stimulation (TMS). Although TMS is safe and relatively easy to administer, its efficacy has still to be definitively established. Other modalities, at various stages of research development, include magnetic seizure therapy (MST), deep brain stimulation (DBS), and vagus nerve stimulation (VNS). We briefly review the development and technical aspects of these treatments, their potential role in the treatment of major depression, adverse effects, and putative mechanism of action. As the only one of these treatment modalities that is in widespread clinical use, more extended consideration is given to ECT Although more than half a century has elapsed since ECT was first introduced, it remains the most effective treatment for major depression, with efficacy in patients refractory to antidepressant drugs and an acceptable safety profile. Although they hold considerable promise, the novel brain stimulation techniques reviewed here will be need to be further developed before they achieve clinical acceptability.	topic_bd
77708	4	356169	7	NULL	NULL	0	NULL	TMS	MedicalProcedure		is					transcranial magnetic stimulation 	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Until recently, a review of nonpharmacological, somatic treatments of psychiatric disorders would have included only electroconvulsive therapy (ECT). This situation is now changing very substantially. Although ECT remains the only modality in widespread clinical use, several new techniques are under investigation. Their principal indication in the psychiatric context is the treatment of major depression, but other applications are also being studied. All the novel treatments involve brain stimulation, which is achieved by different technological methods. The treatment closest to the threshold of clinical acceptability is transcranial magnetic stimulation (TMS). Although TMS is safe and relatively easy to administer, its efficacy has still to be definitively established. Other modalities, at various stages of research development, include magnetic seizure therapy (MST), deep brain stimulation (DBS), and vagus nerve stimulation (VNS). We briefly review the development and technical aspects of these treatments, their potential role in the treatment of major depression, adverse effects, and putative mechanism of action. As the only one of these treatment modalities that is in widespread clinical use, more extended consideration is given to ECT Although more than half a century has elapsed since ECT was first introduced, it remains the most effective treatment for major depression, with efficacy in patients refractory to antidepressant drugs and an acceptable safety profile. Although they hold considerable promise, the novel brain stimulation techniques reviewed here will be need to be further developed before they achieve clinical acceptability.	topic_bd
77709	5	356169	7	NULL	NULL	0	NULL	MST	MedicalProcedure		is used in the					major depression	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	Until recently, a review of nonpharmacological, somatic treatments of psychiatric disorders would have included only electroconvulsive therapy (ECT). This situation is now changing very substantially. Although ECT remains the only modality in widespread clinical use, several new techniques are under investigation. Their principal indication in the psychiatric context is the treatment of major depression, but other applications are also being studied. All the novel treatments involve brain stimulation, which is achieved by different technological methods. The treatment closest to the threshold of clinical acceptability is transcranial magnetic stimulation (TMS). Although TMS is safe and relatively easy to administer, its efficacy has still to be definitively established. Other modalities, at various stages of research development, include magnetic seizure therapy (MST), deep brain stimulation (DBS), and vagus nerve stimulation (VNS). We briefly review the development and technical aspects of these treatments, their potential role in the treatment of major depression, adverse effects, and putative mechanism of action. As the only one of these treatment modalities that is in widespread clinical use, more extended consideration is given to ECT Although more than half a century has elapsed since ECT was first introduced, it remains the most effective treatment for major depression, with efficacy in patients refractory to antidepressant drugs and an acceptable safety profile. Although they hold considerable promise, the novel brain stimulation techniques reviewed here will be need to be further developed before they achieve clinical acceptability.	topic_bd
77710	6	356169	7	NULL	NULL	0	NULL	MST	MedicalProcedure		is					magnetic seizure therapy	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Until recently, a review of nonpharmacological, somatic treatments of psychiatric disorders would have included only electroconvulsive therapy (ECT). This situation is now changing very substantially. Although ECT remains the only modality in widespread clinical use, several new techniques are under investigation. Their principal indication in the psychiatric context is the treatment of major depression, but other applications are also being studied. All the novel treatments involve brain stimulation, which is achieved by different technological methods. The treatment closest to the threshold of clinical acceptability is transcranial magnetic stimulation (TMS). Although TMS is safe and relatively easy to administer, its efficacy has still to be definitively established. Other modalities, at various stages of research development, include magnetic seizure therapy (MST), deep brain stimulation (DBS), and vagus nerve stimulation (VNS). We briefly review the development and technical aspects of these treatments, their potential role in the treatment of major depression, adverse effects, and putative mechanism of action. As the only one of these treatment modalities that is in widespread clinical use, more extended consideration is given to ECT Although more than half a century has elapsed since ECT was first introduced, it remains the most effective treatment for major depression, with efficacy in patients refractory to antidepressant drugs and an acceptable safety profile. Although they hold considerable promise, the novel brain stimulation techniques reviewed here will be need to be further developed before they achieve clinical acceptability.	topic_bd
77711	7	356169	7	NULL	NULL	0	NULL	DBS	MedicalProcedure		is used in the					major depression	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	Until recently, a review of nonpharmacological, somatic treatments of psychiatric disorders would have included only electroconvulsive therapy (ECT). This situation is now changing very substantially. Although ECT remains the only modality in widespread clinical use, several new techniques are under investigation. Their principal indication in the psychiatric context is the treatment of major depression, but other applications are also being studied. All the novel treatments involve brain stimulation, which is achieved by different technological methods. The treatment closest to the threshold of clinical acceptability is transcranial magnetic stimulation (TMS). Although TMS is safe and relatively easy to administer, its efficacy has still to be definitively established. Other modalities, at various stages of research development, include magnetic seizure therapy (MST), deep brain stimulation (DBS), and vagus nerve stimulation (VNS). We briefly review the development and technical aspects of these treatments, their potential role in the treatment of major depression, adverse effects, and putative mechanism of action. As the only one of these treatment modalities that is in widespread clinical use, more extended consideration is given to ECT Although more than half a century has elapsed since ECT was first introduced, it remains the most effective treatment for major depression, with efficacy in patients refractory to antidepressant drugs and an acceptable safety profile. Although they hold considerable promise, the novel brain stimulation techniques reviewed here will be need to be further developed before they achieve clinical acceptability.	topic_bd
77712	8	356169	7	NULL	NULL	0	NULL	DBS	MedicalProcedure		is					deep brain stimulation	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Until recently, a review of nonpharmacological, somatic treatments of psychiatric disorders would have included only electroconvulsive therapy (ECT). This situation is now changing very substantially. Although ECT remains the only modality in widespread clinical use, several new techniques are under investigation. Their principal indication in the psychiatric context is the treatment of major depression, but other applications are also being studied. All the novel treatments involve brain stimulation, which is achieved by different technological methods. The treatment closest to the threshold of clinical acceptability is transcranial magnetic stimulation (TMS). Although TMS is safe and relatively easy to administer, its efficacy has still to be definitively established. Other modalities, at various stages of research development, include magnetic seizure therapy (MST), deep brain stimulation (DBS), and vagus nerve stimulation (VNS). We briefly review the development and technical aspects of these treatments, their potential role in the treatment of major depression, adverse effects, and putative mechanism of action. As the only one of these treatment modalities that is in widespread clinical use, more extended consideration is given to ECT Although more than half a century has elapsed since ECT was first introduced, it remains the most effective treatment for major depression, with efficacy in patients refractory to antidepressant drugs and an acceptable safety profile. Although they hold considerable promise, the novel brain stimulation techniques reviewed here will be need to be further developed before they achieve clinical acceptability.	topic_bd
77713	9	356169	7	NULL	NULL	0	NULL	VNS	MedicalProcedure		is used in the					major depression	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	Until recently, a review of nonpharmacological, somatic treatments of psychiatric disorders would have included only electroconvulsive therapy (ECT). This situation is now changing very substantially. Although ECT remains the only modality in widespread clinical use, several new techniques are under investigation. Their principal indication in the psychiatric context is the treatment of major depression, but other applications are also being studied. All the novel treatments involve brain stimulation, which is achieved by different technological methods. The treatment closest to the threshold of clinical acceptability is transcranial magnetic stimulation (TMS). Although TMS is safe and relatively easy to administer, its efficacy has still to be definitively established. Other modalities, at various stages of research development, include magnetic seizure therapy (MST), deep brain stimulation (DBS), and vagus nerve stimulation (VNS). We briefly review the development and technical aspects of these treatments, their potential role in the treatment of major depression, adverse effects, and putative mechanism of action. As the only one of these treatment modalities that is in widespread clinical use, more extended consideration is given to ECT Although more than half a century has elapsed since ECT was first introduced, it remains the most effective treatment for major depression, with efficacy in patients refractory to antidepressant drugs and an acceptable safety profile. Although they hold considerable promise, the novel brain stimulation techniques reviewed here will be need to be further developed before they achieve clinical acceptability.	topic_bd
77714	10	356169	7	NULL	NULL	0	NULL	VNS	MedicalProcedure		is					vagus nerve stimulation 	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Until recently, a review of nonpharmacological, somatic treatments of psychiatric disorders would have included only electroconvulsive therapy (ECT). This situation is now changing very substantially. Although ECT remains the only modality in widespread clinical use, several new techniques are under investigation. Their principal indication in the psychiatric context is the treatment of major depression, but other applications are also being studied. All the novel treatments involve brain stimulation, which is achieved by different technological methods. The treatment closest to the threshold of clinical acceptability is transcranial magnetic stimulation (TMS). Although TMS is safe and relatively easy to administer, its efficacy has still to be definitively established. Other modalities, at various stages of research development, include magnetic seizure therapy (MST), deep brain stimulation (DBS), and vagus nerve stimulation (VNS). We briefly review the development and technical aspects of these treatments, their potential role in the treatment of major depression, adverse effects, and putative mechanism of action. As the only one of these treatment modalities that is in widespread clinical use, more extended consideration is given to ECT Although more than half a century has elapsed since ECT was first introduced, it remains the most effective treatment for major depression, with efficacy in patients refractory to antidepressant drugs and an acceptable safety profile. Although they hold considerable promise, the novel brain stimulation techniques reviewed here will be need to be further developed before they achieve clinical acceptability.	topic_bd
78317	1	356197	5	NULL	NULL	0	NULL	microglia	Cell	stimulation of	leads to					positive-feedback loop	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Microglia and astrocyte stimulation lead to a positive-feedback loop that also facilitates the development of a chronic inflammatory environment within the fetus, pre-disposing it to lifelong comorbid psychiatric and systemic pathologies	topic_aut
78318	2	356197	5	NULL	NULL	NULL	NULL	statement 1	Process		facilitates					chronic inflammatory environment	AbstractConcept	development of			NULL	within fetus	NULL	NULL	NULL	NULL	NULL	NULL	Microglia and astrocyte stimulation lead to a positive-feedback loop that also facilitates the development of a chronic inflammatory environment within the fetus, pre-disposing it to lifelong comorbid psychiatric and systemic pathologies	topic_aut
78319	3	356197	5	NULL	NULL	0	NULL	fetus	OrganismPart		is pre-disposed to					comorbid psychiatric pathologies	MedicalFinding	lifelong			NULL		0	NULL	NULL	NULL	NULL	NULL	Microglia and astrocyte stimulation lead to a positive-feedback loop that also facilitates the development of a chronic inflammatory environment within the fetus, pre-disposing it to lifelong comorbid psychiatric and systemic pathologies	topic_aut
78320	4	356197	5	NULL	NULL	0	NULL	statement 2	Process		leads to					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Microglia and astrocyte stimulation lead to a positive-feedback loop that also facilitates the development of a chronic inflammatory environment within the fetus, pre-disposing it to lifelong comorbid psychiatric and systemic pathologies	topic_aut
78321	5	356197	5	NULL	NULL	0	NULL	fetus	OrganismPart		is pre-disposed to					systemic pathologies	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Microglia and astrocyte stimulation lead to a positive-feedback loop that also facilitates the development of a chronic inflammatory environment within the fetus, pre-disposing it to lifelong comorbid psychiatric and systemic pathologies	topic_aut
78322	6	356197	5	NULL	NULL	0	NULL	statement 2	Process		leads to					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Microglia and astrocyte stimulation lead to a positive-feedback loop that also facilitates the development of a chronic inflammatory environment within the fetus, pre-disposing it to lifelong comorbid psychiatric and systemic pathologies	topic_aut
78323	7	356197	5	NULL	NULL	0	NULL	astrocyte	Cell	stimulation of	leads to					positive-feedback loop	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Microglia and astrocyte stimulation lead to a positive-feedback loop that also facilitates the development of a chronic inflammatory environment within the fetus, pre-disposing it to lifelong comorbid psychiatric and systemic pathologies	topic_aut
78324	8	356197	5	NULL	NULL	0	NULL	statement 7	Process		leads to					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Microglia and astrocyte stimulation lead to a positive-feedback loop that also facilitates the development of a chronic inflammatory environment within the fetus, pre-disposing it to lifelong comorbid psychiatric and systemic pathologies	topic_aut
78325	9	356197	5	NULL	NULL	0	NULL	statement 7	Process		leads to					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Microglia and astrocyte stimulation lead to a positive-feedback loop that also facilitates the development of a chronic inflammatory environment within the fetus, pre-disposing it to lifelong comorbid psychiatric and systemic pathologies	topic_aut
78326	1	356198	5	NULL	NULL	0	NULL	autistic individuals	GroupOfPeople		is hyper-sensite to					environmental stimuli	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	NULL	NULL	Such a mechanism could account for many of the observed symptoms and behaviors of autistic individuals such as hyper-sensitivity to environmental stimuli, object fixation, echolalia, repetitive physical behaviors, chronic enterocolitis, autoimmune disease, and, at the extreme, savantism	topic_aut
78327	2	356198	5	NULL	NULL	0	NULL	object fixation	MedicalFinding		is a symptom of					autistic individuals	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Such a mechanism could account for many of the observed symptoms and behaviors of autistic individuals such as hyper-sensitivity to environmental stimuli, object fixation, echolalia, repetitive physical behaviors, chronic enterocolitis, autoimmune disease, and, at the extreme, savantism	topic_aut
78328	3	356198	5	NULL	NULL	0	NULL	echolalia	MedicalFinding		is a symptom of					autistic individuals	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Such a mechanism could account for many of the observed symptoms and behaviors of autistic individuals such as hyper-sensitivity to environmental stimuli, object fixation, echolalia, repetitive physical behaviors, chronic enterocolitis, autoimmune disease, and, at the extreme, savantism	topic_aut
78329	4	356198	5	NULL	NULL	0	NULL	repetitive physical behaviors	MedicalFinding		is a symptom of					autistic individuals	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Such a mechanism could account for many of the observed symptoms and behaviors of autistic individuals such as hyper-sensitivity to environmental stimuli, object fixation, echolalia, repetitive physical behaviors, chronic enterocolitis, autoimmune disease, and, at the extreme, savantism	topic_aut
78330	5	356198	5	NULL	NULL	0	NULL	chronic enterocolitis	MedicalFinding		is a symptom of					autistic individuals	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Such a mechanism could account for many of the observed symptoms and behaviors of autistic individuals such as hyper-sensitivity to environmental stimuli, object fixation, echolalia, repetitive physical behaviors, chronic enterocolitis, autoimmune disease, and, at the extreme, savantism	topic_aut
78331	6	356198	5	NULL	NULL	0	NULL	autoimmune disease	MedicalFinding		is a symptom of					autistic individuals	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Such a mechanism could account for many of the observed symptoms and behaviors of autistic individuals such as hyper-sensitivity to environmental stimuli, object fixation, echolalia, repetitive physical behaviors, chronic enterocolitis, autoimmune disease, and, at the extreme, savantism	topic_aut
78332	7	356198	5	NULL	NULL	0	NULL	savantism	MedicalFinding		is a symptom of					autistic individuals	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Such a mechanism could account for many of the observed symptoms and behaviors of autistic individuals such as hyper-sensitivity to environmental stimuli, object fixation, echolalia, repetitive physical behaviors, chronic enterocolitis, autoimmune disease, and, at the extreme, savantism	topic_aut
78333	1	356199	5	NULL	NULL	NULL	NULL	vocalizations	Process		repeated by		automatically			another person	GroupOfPeople				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Echolalia is the automatic repetition of vocalizations made by another person. It is closely related to echopraxia, the automatic repetition of movements made by another person.	topic_aut
78334	2	356199	5	NULL	NULL	NULL	NULL	statement 1	Process		is termed as					Echolalia	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Echolalia is the automatic repetition of vocalizations made by another person. It is closely related to echopraxia, the automatic repetition of movements made by another person.	topic_aut
78335	3	356199	5	NULL	NULL	NULL	NULL	echolalia	MedicalFinding		is related to		closely			echopraxia	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Echolalia is the automatic repetition of vocalizations made by another person. It is closely related to echopraxia, the automatic repetition of movements made by another person.	topic_aut
78336	4	356199	5	NULL	NULL	0	NULL	movements	PhysicalPhenomenon		repeated by		automatically			another person	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Echolalia is the automatic repetition of vocalizations made by another person. It is closely related to echopraxia, the automatic repetition of movements made by another person.	topic_aut
78337	5	356199	5	NULL	NULL	0	NULL	statement 4	Process		is termed as					echopraxia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Echolalia is the automatic repetition of vocalizations made by another person. It is closely related to echopraxia, the automatic repetition of movements made by another person.	topic_aut
78338	1	356200	5	NULL	NULL	0	NULL	colon	OrganismPart	inflammation of	is known as					enterocolitis 	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Enterocolitis (or 'coloenteritis') is an inflammation of the colon and small intestine.[1] However, most conditions are categorized as one or the other of the following:	topic_aut
78339	2	356200	5	NULL	NULL	0	NULL	small intestine	OrganismPart	inflammation of	is known as					enterocolitis	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Enterocolitis (or 'coloenteritis') is an inflammation of the colon and small intestine.[1] However, most conditions are categorized as one or the other of the following:	topic_aut
78340	3	356200	5	NULL	NULL	0	NULL	coloenteritis	MedicalFinding		is also known as					enterocolitis	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Enterocolitis (or 'coloenteritis') is an inflammation of the colon and small intestine.[1] However, most conditions are categorized as one or the other of the following:	topic_aut
78348	1	356202	5	NULL	NULL	0	NULL	pathogens	Organism	prenatal exposure to	corelates with		significantly			ASD	MedicalFinding	occurence of			NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiological data has highlighted this relationship showing significant correlations between prenatal exposure to pathogens, including influenza, and the occurrence of ASD	topic_aut
78349	1	356203	5	NULL	NULL	0	NULL	MIA	Process		is					maternal immune activation	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Several groups utilizing these animal models have found that activation of the maternal immune system, termed maternal immune activation (MIA), and more specifically the exposure of the developing fetus to maternal cytokines precipitate the neurological, immunological and behavioral abnormalities observed in the offspring of these animals	topic_aut
78350	2	356203	5	NULL	NULL	0	NULL	maternal immune system	Process	activated	is termed as					MIA	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Several groups utilizing these animal models have found that activation of the maternal immune system, termed maternal immune activation (MIA), and more specifically the exposure of the developing fetus to maternal cytokines precipitate the neurological, immunological and behavioral abnormalities observed in the offspring of these animals	topic_aut
78351	3	356203	5	NULL	NULL	0	NULL	statement 2	Process		precipitate					neurological abnormalities	MedicalFinding				NULL	animal offsprings	0	NULL	NULL	NULL	NULL	NULL	Several groups utilizing these animal models have found that activation of the maternal immune system, termed maternal immune activation (MIA), and more specifically the exposure of the developing fetus to maternal cytokines precipitate the neurological, immunological and behavioral abnormalities observed in the offspring of these animals	topic_aut
78352	4	356203	5	NULL	NULL	0	NULL	statement 2	Process		precipitate					immunological abnormalities	MedicalFinding				NULL	animal offsprings	0	NULL	NULL	NULL	NULL	NULL	Several groups utilizing these animal models have found that activation of the maternal immune system, termed maternal immune activation (MIA), and more specifically the exposure of the developing fetus to maternal cytokines precipitate the neurological, immunological and behavioral abnormalities observed in the offspring of these animals	topic_aut
78353	5	356203	5	NULL	NULL	0	NULL	statement 2	Process		precipitate					behavioral abnormalities	MedicalFinding				NULL	animal offsprings	0	NULL	NULL	NULL	NULL	NULL	Several groups utilizing these animal models have found that activation of the maternal immune system, termed maternal immune activation (MIA), and more specifically the exposure of the developing fetus to maternal cytokines precipitate the neurological, immunological and behavioral abnormalities observed in the offspring of these animals	topic_aut
78354	6	356203	5	NULL	NULL	0	NULL	fetus	OrganismPart	developing	is exposed to					cytokines	GP	maternal			NULL		0	NULL	NULL	NULL	NULL	NULL	Several groups utilizing these animal models have found that activation of the maternal immune system, termed maternal immune activation (MIA), and more specifically the exposure of the developing fetus to maternal cytokines precipitate the neurological, immunological and behavioral abnormalities observed in the offspring of these animals	topic_aut
78355	7	356203	5	NULL	NULL	0	NULL	statement 6	Process		precipitate					neurological abnormalities	MedicalFinding				NULL	animal offsprings	0	NULL	NULL	NULL	NULL	NULL	Several groups utilizing these animal models have found that activation of the maternal immune system, termed maternal immune activation (MIA), and more specifically the exposure of the developing fetus to maternal cytokines precipitate the neurological, immunological and behavioral abnormalities observed in the offspring of these animals	topic_aut
78356	8	356203	5	NULL	NULL	0	NULL	statement 6	Process		precipitate					immunological abnormalities	MedicalFinding				NULL	animal offsprings	0	NULL	NULL	NULL	NULL	NULL	Several groups utilizing these animal models have found that activation of the maternal immune system, termed maternal immune activation (MIA), and more specifically the exposure of the developing fetus to maternal cytokines precipitate the neurological, immunological and behavioral abnormalities observed in the offspring of these animals	topic_aut
78357	9	356203	5	NULL	NULL	0	NULL	statement 6	Process		precipitate					behavioral abnormalities	MedicalFinding				NULL	animal offsprings	0	NULL	NULL	NULL	NULL	NULL	Several groups utilizing these animal models have found that activation of the maternal immune system, termed maternal immune activation (MIA), and more specifically the exposure of the developing fetus to maternal cytokines precipitate the neurological, immunological and behavioral abnormalities observed in the offspring of these animals	topic_aut
78358	1	356204	5	NULL	NULL	NULL	NULL	autism spectrum conditions	MedicalFinding		is an exaggeration of					low-empathizing behaviors	MedicalFinding	normal;;male			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Autism spectrum conditions have been hypothesized to be an exaggeration of normal male low-empathizing and high-systemizing behaviors.	topic_aut
78359	2	356204	5	NULL	NULL	0	NULL	autism spectrum conditions	MedicalFinding		is an exaggeration of					high-systemizing behavior	MedicalFinding	normal;;male			NULL		0	NULL	NULL	NULL	NULL	NULL	Autism spectrum conditions have been hypothesized to be an exaggeration of normal male low-empathizing and high-systemizing behaviors.	topic_aut
78360	1	356206	5	NULL	NULL	0	NULL	cytokines	GP	levels of	is increased in					AS	MedicalFinding	male			NULL		0	NULL	NULL	NULL	NULL	NULL	Males with AS showed altered levels of 24 biomarkers including increased levels of cytokines and other inflammatory molecules	topic_aut
78361	2	356206	5	NULL	NULL	0	NULL	inflammatory molecules	GP	levels of	is increased in					AS	MedicalFinding	male			NULL		0	NULL	NULL	NULL	NULL	NULL	Males with AS showed altered levels of 24 biomarkers including increased levels of cytokines and other inflammatory molecules	topic_aut
78362	1	356207	5	NULL	NULL	0	NULL	testosterone	GP		is elevated in					AS	MedicalFinding	females			NULL		0	NULL	NULL	NULL	NULL	NULL	The finding of elevated testosterone in AS females confirmed predictions from the 'extreme male brain' and androgen theories of autism spectrum conditions	topic_aut
78377	1	356208	5	NULL	NULL	0	NULL	cellular immune function	Process	altered;;adaptive	is present in					ASD children	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Overall these data indicate significantly altered adaptive cellular immune function in children with ASD that may reflect dysfunctional immune activation, along with evidence that these perturbations may be linked to disturbances in behavior and developmental functioning	topic_aut
78378	2	356208	5	NULL	NULL	0	NULL	statement 1	Process		reflects		may			immune activation	Process	dysfunctional			NULL		0	NULL	NULL	NULL	NULL	NULL	Overall these data indicate significantly altered adaptive cellular immune function in children with ASD that may reflect dysfunctional immune activation, along with evidence that these perturbations may be linked to disturbances in behavior and developmental functioning	topic_aut
78379	3	356208	5	NULL	NULL	0	NULL	statement 1	Process		is linked to					behavior	MentalProcess	disturbances in			NULL		0	NULL	NULL	NULL	NULL	NULL	Overall these data indicate significantly altered adaptive cellular immune function in children with ASD that may reflect dysfunctional immune activation, along with evidence that these perturbations may be linked to disturbances in behavior and developmental functioning	topic_aut
78380	4	356208	5	NULL	NULL	0	NULL	statement 1	Process		is linked to					developmental functioning	Process	disturbances in			NULL		0	NULL	NULL	NULL	NULL	NULL	Overall these data indicate significantly altered adaptive cellular immune function in children with ASD that may reflect dysfunctional immune activation, along with evidence that these perturbations may be linked to disturbances in behavior and developmental functioning	topic_aut
78381	1	356209	5	NULL	NULL	0	NULL	TNF-	GP		is a type of					pro-inflammatory cytokines	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	We found increased expression levels of pro-inflammatory cytokines TNF-α and IL-6, but decreased Bcl2 expression in lymphoblasts of autistic subjects.	topic_aut
78382	2	356209	5	NULL	NULL	0	NULL	IL-6	GP		is a type of					pro-inflammatory cytokines	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	We found increased expression levels of pro-inflammatory cytokines TNF-α and IL-6, but decreased Bcl2 expression in lymphoblasts of autistic subjects.	topic_aut
78383	3	356209	5	NULL	NULL	0	NULL	TNF-	GP	expression of	is increased in					autistic subjects	GroupOfPeople	lymphoblasts of			NULL		0	NULL	NULL	NULL	NULL	NULL	We found increased expression levels of pro-inflammatory cytokines TNF-α and IL-6, but decreased Bcl2 expression in lymphoblasts of autistic subjects.	topic_aut
78384	4	356209	5	NULL	NULL	0	NULL	IL-6	GP	expression of	is increased in					autistic subjects	GroupOfPeople	lymphoblasts of			NULL		0	NULL	NULL	NULL	NULL	NULL	We found increased expression levels of pro-inflammatory cytokines TNF-α and IL-6, but decreased Bcl2 expression in lymphoblasts of autistic subjects.	topic_aut
78385	5	356209	5	NULL	NULL	0	NULL	Bcl2	GP	expression of	decreased in					autistic subjects	GroupOfPeople	lymphoblasts of			NULL		0	NULL	NULL	NULL	NULL	NULL	We found increased expression levels of pro-inflammatory cytokines TNF-α and IL-6, but decreased Bcl2 expression in lymphoblasts of autistic subjects.	topic_aut
78386	1	356210	5	NULL	NULL	NULL	NULL	maternal infection	MedicalFinding	human	occurs during					pregnancy	Process	human			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Epidemiological studies with human populations indicate associations between maternal infection during pregnancy and increased risk in offspring for central nervous system (CNS) disorders including schizophrenia, autism and cerebral palsy.	topic_aut
78387	2	356210	5	NULL	NULL	0	NULL	statement 1	Process		increases					schizophrenia	MedicalFinding	risk of;;offspring			NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiological studies with human populations indicate associations between maternal infection during pregnancy and increased risk in offspring for central nervous system (CNS) disorders including schizophrenia, autism and cerebral palsy.	topic_aut
78388	3	356210	5	NULL	NULL	0	NULL	statement 1	Process		increases					autism	MedicalFinding	risk of;;offspring			NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiological studies with human populations indicate associations between maternal infection during pregnancy and increased risk in offspring for central nervous system (CNS) disorders including schizophrenia, autism and cerebral palsy.	topic_aut
78389	4	356210	5	NULL	NULL	0	NULL	statement 1	Process		increases					cerebral palsy	MedicalFinding	risk of;;childhood			NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiological studies with human populations indicate associations between maternal infection during pregnancy and increased risk in offspring for central nervous system (CNS) disorders including schizophrenia, autism and cerebral palsy.	topic_aut
78390	5	356210	5	NULL	NULL	0	NULL	schizophrenia	MedicalFinding		is a type of					CNS disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiological studies with human populations indicate associations between maternal infection during pregnancy and increased risk in offspring for central nervous system (CNS) disorders including schizophrenia, autism and cerebral palsy.	topic_aut
78391	6	356210	5	NULL	NULL	0	NULL	autism	MedicalFinding		is a type of					CNS disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiological studies with human populations indicate associations between maternal infection during pregnancy and increased risk in offspring for central nervous system (CNS) disorders including schizophrenia, autism and cerebral palsy.	topic_aut
78392	7	356210	5	NULL	NULL	0	NULL	cerebral palsy	MedicalFinding		is a type of					CNS disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiological studies with human populations indicate associations between maternal infection during pregnancy and increased risk in offspring for central nervous system (CNS) disorders including schizophrenia, autism and cerebral palsy.	topic_aut
78393	8	356210	5	NULL	NULL	0	NULL	CNS disorder	MedicalFinding		is					central nervous system disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiological studies with human populations indicate associations between maternal infection during pregnancy and increased risk in offspring for central nervous system (CNS) disorders including schizophrenia, autism and cerebral palsy.	topic_aut
78394	1	356212	5	NULL	NULL	0	NULL	ASD	MedicalFinding		is					autism spectrum disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Many patients with Autism Spectrum Disorders (ASD) have "allergic" symptoms; moreover, the prevalence of ASD in patients with mastocytosis, characterized by numerous hyperactive mast cells in most tissues, is 10-fold higher than the general population suggesting mast cell involvement	topic_aut
78395	2	356212	5	NULL	NULL	0	NULL	ASD patients	GroupOfPeople		is prevalent in					mastocytosis	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Many patients with Autism Spectrum Disorders (ASD) have "allergic" symptoms; moreover, the prevalence of ASD in patients with mastocytosis, characterized by numerous hyperactive mast cells in most tissues, is 10-fold higher than the general population suggesting mast cell involvement	topic_aut
78396	3	356212	5	NULL	NULL	0	NULL	mastocytosis	MedicalFinding		is characterized by					mast cells	Cell	numerous;;hyperactive			NULL	most tissues	0	NULL	NULL	NULL	NULL	NULL	Many patients with Autism Spectrum Disorders (ASD) have "allergic" symptoms; moreover, the prevalence of ASD in patients with mastocytosis, characterized by numerous hyperactive mast cells in most tissues, is 10-fold higher than the general population suggesting mast cell involvement	topic_aut
78397	1	356213	5	NULL	NULL	NULL	NULL	blood-brain-barrier	PhysicalPhenomenon	disruption of	permit					brain inflammation	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	This phenomenon could disrupt the blood-brain-barrier and permit brain inflammation	topic_aut
78398	1	356214	5	NULL	NULL	0	NULL	VEGF	GP		is released from					mast cells	Cell	human			NULL		0	NULL	NULL	NULL	NULL	NULL	HgCl2 stimulates VEGF and IL-6 release from human mast cells. This phenomenon could disrupt the blood-brain-barrier and permit brain inflammation.	topic_aut
78399	2	356214	5	NULL	NULL	0	NULL	IL-6	GP		is released from					mast cells	Cell	human			NULL		0	NULL	NULL	NULL	NULL	NULL	HgCl2 stimulates VEGF and IL-6 release from human mast cells. This phenomenon could disrupt the blood-brain-barrier and permit brain inflammation.	topic_aut
78400	3	356214	5	NULL	NULL	0	NULL	HgCl2	Chemical		stimulates					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	HgCl2 stimulates VEGF and IL-6 release from human mast cells. This phenomenon could disrupt the blood-brain-barrier and permit brain inflammation.	topic_aut
78401	4	356214	5	NULL	NULL	0	NULL	HgCl2	Chemical		stimulates					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	HgCl2 stimulates VEGF and IL-6 release from human mast cells. This phenomenon could disrupt the blood-brain-barrier and permit brain inflammation.	topic_aut
78402	5	356214	5	NULL	NULL	0	NULL	statement 3	Process		disrupt					blood-brain-barrier	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	NULL	NULL	HgCl2 stimulates VEGF and IL-6 release from human mast cells. This phenomenon could disrupt the blood-brain-barrier and permit brain inflammation.	topic_aut
78403	6	356214	5	NULL	NULL	0	NULL	statement 5	Process		permit					brain inflammation	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	HgCl2 stimulates VEGF and IL-6 release from human mast cells. This phenomenon could disrupt the blood-brain-barrier and permit brain inflammation.	topic_aut
78404	7	356214	5	NULL	NULL	0	NULL	statement 4	Process		disrupt					blood-brain-barrier	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	NULL	NULL	HgCl2 stimulates VEGF and IL-6 release from human mast cells. This phenomenon could disrupt the blood-brain-barrier and permit brain inflammation.	topic_aut
78405	8	356214	5	NULL	NULL	0	NULL	statement 7	Process		permit					brain inflammation	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	HgCl2 stimulates VEGF and IL-6 release from human mast cells. This phenomenon could disrupt the blood-brain-barrier and permit brain inflammation.	topic_aut
78406	1	356215	5	NULL	NULL	0	NULL	IL-1	GP		mediates					placental damage	MedicalFinding				NULL	offspring	0	NULL	NULL	NULL	NULL	NULL	In this study, we demonstrate that IL-1 plays a key role in mediating severe placental damage and neurodevelopmental anomalies in offspring.	topic_aut
78407	2	356215	5	NULL	NULL	0	NULL	IL-1	GP		mediates					neurodevelopmental anomalies	MedicalFinding				NULL	offspring	0	NULL	NULL	NULL	NULL	NULL	In this study, we demonstrate that IL-1 plays a key role in mediating severe placental damage and neurodevelopmental anomalies in offspring.	topic_aut
78408	1	356216	5	NULL	NULL	0	NULL	rats	Organism	gestation exposure of;;pregnant	exposed to					LPS	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that end of gestation exposure of pregnant rats to systemic microbial product (LPS) triggers placental inflammation and massive cell death, fetal mortality, and both forebrain white matter and motor behavioral alterations in the offspring	topic_aut
78409	2	356216	5	NULL	NULL	0	NULL	LPS	Chemical		is a type of					systemic microbial product	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that end of gestation exposure of pregnant rats to systemic microbial product (LPS) triggers placental inflammation and massive cell death, fetal mortality, and both forebrain white matter and motor behavioral alterations in the offspring	topic_aut
78410	3	356216	5	NULL	NULL	0	NULL	statement 1	Process		trigger					placental inflammation	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that end of gestation exposure of pregnant rats to systemic microbial product (LPS) triggers placental inflammation and massive cell death, fetal mortality, and both forebrain white matter and motor behavioral alterations in the offspring	topic_aut
78411	4	356216	5	NULL	NULL	0	NULL	statement 1	Process		trigger					cell death	MedicalFinding	massive			NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that end of gestation exposure of pregnant rats to systemic microbial product (LPS) triggers placental inflammation and massive cell death, fetal mortality, and both forebrain white matter and motor behavioral alterations in the offspring	topic_aut
78412	5	356216	5	NULL	NULL	0	NULL	statement 1	Process		trigger					fetal mortality	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that end of gestation exposure of pregnant rats to systemic microbial product (LPS) triggers placental inflammation and massive cell death, fetal mortality, and both forebrain white matter and motor behavioral alterations in the offspring	topic_aut
78413	6	356216	5	NULL	NULL	0	NULL	statement 1	Process		trigger					behavioral alterations	MedicalFinding	forebrain white matter			NULL	offspring	0	NULL	NULL	NULL	NULL	NULL	Our results show that end of gestation exposure of pregnant rats to systemic microbial product (LPS) triggers placental inflammation and massive cell death, fetal mortality, and both forebrain white matter and motor behavioral alterations in the offspring	topic_aut
78414	7	356216	5	NULL	NULL	0	NULL	statement 1	Process		trigger					behavioral alterations	MedicalFinding	motor			NULL	offspring	0	NULL	NULL	NULL	NULL	NULL	Our results show that end of gestation exposure of pregnant rats to systemic microbial product (LPS) triggers placental inflammation and massive cell death, fetal mortality, and both forebrain white matter and motor behavioral alterations in the offspring	topic_aut
77715	1	356218	7	NULL	NULL	0	NULL	GIV 	GP		is a type of					metastasis-related protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Here we identify GIV as a metastasis-related protein whose full-length transcript (GIV-fl) is expressed exclusively in highly invasive colon, breast, and pancreatic carcinoma cells and not in their poorly invasive counterparts.	topic_ccc
77716	2	356218	7	NULL	NULL	NULL	NULL	GIV-fl	GP		expressed in		exclusively			colon carcinoma cells	Cell	highly invasive			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we identify GIV as a metastasis-related protein whose full-length transcript (GIV-fl) is expressed exclusively in highly invasive colon, breast, and pancreatic carcinoma cells and not in their poorly invasive counterparts.	topic_ccc
77717	3	356218	7	NULL	NULL	0	NULL	GIV-fl	GP		expressed in		exclusively			breast carcinoma cells	Cell	highly invasive			NULL		0	NULL	NULL	NULL	NULL	NULL	Here we identify GIV as a metastasis-related protein whose full-length transcript (GIV-fl) is expressed exclusively in highly invasive colon, breast, and pancreatic carcinoma cells and not in their poorly invasive counterparts.	topic_ccc
77718	4	356218	7	NULL	NULL	NULL	NULL	GIV-fl	GP		expressed in		exclusively			pancreatic carcinoma cells	Cell	highly invasive			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we identify GIV as a metastasis-related protein whose full-length transcript (GIV-fl) is expressed exclusively in highly invasive colon, breast, and pancreatic carcinoma cells and not in their poorly invasive counterparts.	topic_ccc
77719	5	356218	7	NULL	NULL	0	NULL	GIV-fl	GP		not expressed in					poorly invasive cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Here we identify GIV as a metastasis-related protein whose full-length transcript (GIV-fl) is expressed exclusively in highly invasive colon, breast, and pancreatic carcinoma cells and not in their poorly invasive counterparts.	topic_ccc
77720	6	356218	7	NULL	NULL	0	NULL	GIV-fl	GP		is					GIV full-length transcript	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Here we identify GIV as a metastasis-related protein whose full-length transcript (GIV-fl) is expressed exclusively in highly invasive colon, breast, and pancreatic carcinoma cells and not in their poorly invasive counterparts.	topic_ccc
77721	1	356219	7	NULL	NULL	0	NULL	serotonin signaling	Process	dysfunction of	involved in					SCZ	MedicalFinding	pathogenesis of			NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence indicate that dysfunction of serotonin signaling and HTR2A receptor are involved in the pathogenesis of schizophrenia (SCZ) and bipolar disorder (BD). DNA methylation of HTR2A at T102C polymorphic site influences HTR2A expression and aberrant DNA methylation of HTR2A promoter was reported in postmortem brain of patients with SCZ and BD. Hypothesizing that the brain's epigenetic alteration of HTR2A may also exist in peripheral tissues that can be used as a diagnostic/therapeutic biomarker, we analyzed HTR2A promoter DNA methylation in DNA extracted from the saliva of patients with SCZ and BD, and their first degree relatives versus normal controls. Bisulfite sequencing was used to screen DNA methylation status of the HTR2A promoter CpGs and qMSP was used to quantify the degree of cytosine methylation at differentially methylated sites. Most of the cytosines of the HTR2A promoter were unmethylated. However, CpGs of the -1438A/G polymorphism site, -1420 and -1223 were >95% methylated. The CpG at T102C polymorphic site and neighboring CpGs were ∼70% methylated both in the patients and controls. qMSP analysis revealed that the cytosine of the T102C polymorphic site was significantly hypo-methylated in SCZ, BD, and their first degree relatives compared to the controls. Cytosine methylation of HTR2A at T102C polymorphic site in DNA derived from the saliva can potentially be used as a diagnostic, prognostic, and/or therapeutic biomarker in SCZ and BD. However, these preliminary observations need to be replicated in other populations with a larger sample size to be considered for clinical applications. © 2011 Wiley-Liss, Inc.	topic_bd
77722	2	356219	7	NULL	NULL	NULL	NULL	HTR2A receptor	GP	dysfunction of	involved in					SCZ	MedicalFinding	pathogenesis of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Several lines of evidence indicate that dysfunction of serotonin signaling and HTR2A receptor are involved in the pathogenesis of schizophrenia (SCZ) and bipolar disorder (BD). DNA methylation of HTR2A at T102C polymorphic site influences HTR2A expression and aberrant DNA methylation of HTR2A promoter was reported in postmortem brain of patients with SCZ and BD. Hypothesizing that the brain's epigenetic alteration of HTR2A may also exist in peripheral tissues that can be used as a diagnostic/therapeutic biomarker, we analyzed HTR2A promoter DNA methylation in DNA extracted from the saliva of patients with SCZ and BD, and their first degree relatives versus normal controls. Bisulfite sequencing was used to screen DNA methylation status of the HTR2A promoter CpGs and qMSP was used to quantify the degree of cytosine methylation at differentially methylated sites. Most of the cytosines of the HTR2A promoter were unmethylated. However, CpGs of the -1438A/G polymorphism site, -1420 and -1223 were >95% methylated. The CpG at T102C polymorphic site and neighboring CpGs were ∼70% methylated both in the patients and controls. qMSP analysis revealed that the cytosine of the T102C polymorphic site was significantly hypo-methylated in SCZ, BD, and their first degree relatives compared to the controls. Cytosine methylation of HTR2A at T102C polymorphic site in DNA derived from the saliva can potentially be used as a diagnostic, prognostic, and/or therapeutic biomarker in SCZ and BD. However, these preliminary observations need to be replicated in other populations with a larger sample size to be considered for clinical applications. © 2011 Wiley-Liss, Inc.	topic_bd
77723	3	356219	7	NULL	NULL	NULL	NULL	serotonin signaling	Process	dysfunction of	involved in					BD	MedicalFinding	pathogenesis of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Several lines of evidence indicate that dysfunction of serotonin signaling and HTR2A receptor are involved in the pathogenesis of schizophrenia (SCZ) and bipolar disorder (BD). DNA methylation of HTR2A at T102C polymorphic site influences HTR2A expression and aberrant DNA methylation of HTR2A promoter was reported in postmortem brain of patients with SCZ and BD. Hypothesizing that the brain's epigenetic alteration of HTR2A may also exist in peripheral tissues that can be used as a diagnostic/therapeutic biomarker, we analyzed HTR2A promoter DNA methylation in DNA extracted from the saliva of patients with SCZ and BD, and their first degree relatives versus normal controls. Bisulfite sequencing was used to screen DNA methylation status of the HTR2A promoter CpGs and qMSP was used to quantify the degree of cytosine methylation at differentially methylated sites. Most of the cytosines of the HTR2A promoter were unmethylated. However, CpGs of the -1438A/G polymorphism site, -1420 and -1223 were >95% methylated. The CpG at T102C polymorphic site and neighboring CpGs were ∼70% methylated both in the patients and controls. qMSP analysis revealed that the cytosine of the T102C polymorphic site was significantly hypo-methylated in SCZ, BD, and their first degree relatives compared to the controls. Cytosine methylation of HTR2A at T102C polymorphic site in DNA derived from the saliva can potentially be used as a diagnostic, prognostic, and/or therapeutic biomarker in SCZ and BD. However, these preliminary observations need to be replicated in other populations with a larger sample size to be considered for clinical applications. © 2011 Wiley-Liss, Inc.	topic_bd
77724	4	356219	7	NULL	NULL	0	NULL	HTR2A receptor	GP	dysfunction of	involved in					BD	MedicalFinding	pathogenesis of			NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence indicate that dysfunction of serotonin signaling and HTR2A receptor are involved in the pathogenesis of schizophrenia (SCZ) and bipolar disorder (BD). DNA methylation of HTR2A at T102C polymorphic site influences HTR2A expression and aberrant DNA methylation of HTR2A promoter was reported in postmortem brain of patients with SCZ and BD. Hypothesizing that the brain's epigenetic alteration of HTR2A may also exist in peripheral tissues that can be used as a diagnostic/therapeutic biomarker, we analyzed HTR2A promoter DNA methylation in DNA extracted from the saliva of patients with SCZ and BD, and their first degree relatives versus normal controls. Bisulfite sequencing was used to screen DNA methylation status of the HTR2A promoter CpGs and qMSP was used to quantify the degree of cytosine methylation at differentially methylated sites. Most of the cytosines of the HTR2A promoter were unmethylated. However, CpGs of the -1438A/G polymorphism site, -1420 and -1223 were >95% methylated. The CpG at T102C polymorphic site and neighboring CpGs were ∼70% methylated both in the patients and controls. qMSP analysis revealed that the cytosine of the T102C polymorphic site was significantly hypo-methylated in SCZ, BD, and their first degree relatives compared to the controls. Cytosine methylation of HTR2A at T102C polymorphic site in DNA derived from the saliva can potentially be used as a diagnostic, prognostic, and/or therapeutic biomarker in SCZ and BD. However, these preliminary observations need to be replicated in other populations with a larger sample size to be considered for clinical applications. © 2011 Wiley-Liss, Inc.	topic_bd
77725	5	356219	7	NULL	NULL	0	NULL	HTR2A	GP	DNA methylation of	occur at									T102C polymorphic site 	NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence indicate that dysfunction of serotonin signaling and HTR2A receptor are involved in the pathogenesis of schizophrenia (SCZ) and bipolar disorder (BD). DNA methylation of HTR2A at T102C polymorphic site influences HTR2A expression and aberrant DNA methylation of HTR2A promoter was reported in postmortem brain of patients with SCZ and BD. Hypothesizing that the brain's epigenetic alteration of HTR2A may also exist in peripheral tissues that can be used as a diagnostic/therapeutic biomarker, we analyzed HTR2A promoter DNA methylation in DNA extracted from the saliva of patients with SCZ and BD, and their first degree relatives versus normal controls. Bisulfite sequencing was used to screen DNA methylation status of the HTR2A promoter CpGs and qMSP was used to quantify the degree of cytosine methylation at differentially methylated sites. Most of the cytosines of the HTR2A promoter were unmethylated. However, CpGs of the -1438A/G polymorphism site, -1420 and -1223 were >95% methylated. The CpG at T102C polymorphic site and neighboring CpGs were ∼70% methylated both in the patients and controls. qMSP analysis revealed that the cytosine of the T102C polymorphic site was significantly hypo-methylated in SCZ, BD, and their first degree relatives compared to the controls. Cytosine methylation of HTR2A at T102C polymorphic site in DNA derived from the saliva can potentially be used as a diagnostic, prognostic, and/or therapeutic biomarker in SCZ and BD. However, these preliminary observations need to be replicated in other populations with a larger sample size to be considered for clinical applications. © 2011 Wiley-Liss, Inc.	topic_bd
77726	6	356219	7	NULL	NULL	0	NULL	statement 5	Process		influences					HTR2A	GP	expression of			NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence indicate that dysfunction of serotonin signaling and HTR2A receptor are involved in the pathogenesis of schizophrenia (SCZ) and bipolar disorder (BD). DNA methylation of HTR2A at T102C polymorphic site influences HTR2A expression and aberrant DNA methylation of HTR2A promoter was reported in postmortem brain of patients with SCZ and BD. Hypothesizing that the brain's epigenetic alteration of HTR2A may also exist in peripheral tissues that can be used as a diagnostic/therapeutic biomarker, we analyzed HTR2A promoter DNA methylation in DNA extracted from the saliva of patients with SCZ and BD, and their first degree relatives versus normal controls. Bisulfite sequencing was used to screen DNA methylation status of the HTR2A promoter CpGs and qMSP was used to quantify the degree of cytosine methylation at differentially methylated sites. Most of the cytosines of the HTR2A promoter were unmethylated. However, CpGs of the -1438A/G polymorphism site, -1420 and -1223 were >95% methylated. The CpG at T102C polymorphic site and neighboring CpGs were ∼70% methylated both in the patients and controls. qMSP analysis revealed that the cytosine of the T102C polymorphic site was significantly hypo-methylated in SCZ, BD, and their first degree relatives compared to the controls. Cytosine methylation of HTR2A at T102C polymorphic site in DNA derived from the saliva can potentially be used as a diagnostic, prognostic, and/or therapeutic biomarker in SCZ and BD. However, these preliminary observations need to be replicated in other populations with a larger sample size to be considered for clinical applications. © 2011 Wiley-Liss, Inc.	topic_bd
77727	7	356219	7	NULL	NULL	0	NULL	HTR2A	GP	aberrant DNA methylation of 	reported in				promoter	brain	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence indicate that dysfunction of serotonin signaling and HTR2A receptor are involved in the pathogenesis of schizophrenia (SCZ) and bipolar disorder (BD). DNA methylation of HTR2A at T102C polymorphic site influences HTR2A expression and aberrant DNA methylation of HTR2A promoter was reported in postmortem brain of patients with SCZ and BD. Hypothesizing that the brain's epigenetic alteration of HTR2A may also exist in peripheral tissues that can be used as a diagnostic/therapeutic biomarker, we analyzed HTR2A promoter DNA methylation in DNA extracted from the saliva of patients with SCZ and BD, and their first degree relatives versus normal controls. Bisulfite sequencing was used to screen DNA methylation status of the HTR2A promoter CpGs and qMSP was used to quantify the degree of cytosine methylation at differentially methylated sites. Most of the cytosines of the HTR2A promoter were unmethylated. However, CpGs of the -1438A/G polymorphism site, -1420 and -1223 were >95% methylated. The CpG at T102C polymorphic site and neighboring CpGs were ∼70% methylated both in the patients and controls. qMSP analysis revealed that the cytosine of the T102C polymorphic site was significantly hypo-methylated in SCZ, BD, and their first degree relatives compared to the controls. Cytosine methylation of HTR2A at T102C polymorphic site in DNA derived from the saliva can potentially be used as a diagnostic, prognostic, and/or therapeutic biomarker in SCZ and BD. However, these preliminary observations need to be replicated in other populations with a larger sample size to be considered for clinical applications. © 2011 Wiley-Liss, Inc.	topic_bd
77728	8	356219	7	NULL	NULL	0	NULL	statement 7	Process		occur in					SCZ	MedicalFinding	patients with			NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence indicate that dysfunction of serotonin signaling and HTR2A receptor are involved in the pathogenesis of schizophrenia (SCZ) and bipolar disorder (BD). DNA methylation of HTR2A at T102C polymorphic site influences HTR2A expression and aberrant DNA methylation of HTR2A promoter was reported in postmortem brain of patients with SCZ and BD. Hypothesizing that the brain's epigenetic alteration of HTR2A may also exist in peripheral tissues that can be used as a diagnostic/therapeutic biomarker, we analyzed HTR2A promoter DNA methylation in DNA extracted from the saliva of patients with SCZ and BD, and their first degree relatives versus normal controls. Bisulfite sequencing was used to screen DNA methylation status of the HTR2A promoter CpGs and qMSP was used to quantify the degree of cytosine methylation at differentially methylated sites. Most of the cytosines of the HTR2A promoter were unmethylated. However, CpGs of the -1438A/G polymorphism site, -1420 and -1223 were >95% methylated. The CpG at T102C polymorphic site and neighboring CpGs were ∼70% methylated both in the patients and controls. qMSP analysis revealed that the cytosine of the T102C polymorphic site was significantly hypo-methylated in SCZ, BD, and their first degree relatives compared to the controls. Cytosine methylation of HTR2A at T102C polymorphic site in DNA derived from the saliva can potentially be used as a diagnostic, prognostic, and/or therapeutic biomarker in SCZ and BD. However, these preliminary observations need to be replicated in other populations with a larger sample size to be considered for clinical applications. © 2011 Wiley-Liss, Inc.	topic_bd
77729	9	356219	7	NULL	NULL	0	NULL	statement 7	Process		occur in					BD	MedicalFinding	patients with			NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence indicate that dysfunction of serotonin signaling and HTR2A receptor are involved in the pathogenesis of schizophrenia (SCZ) and bipolar disorder (BD). DNA methylation of HTR2A at T102C polymorphic site influences HTR2A expression and aberrant DNA methylation of HTR2A promoter was reported in postmortem brain of patients with SCZ and BD. Hypothesizing that the brain's epigenetic alteration of HTR2A may also exist in peripheral tissues that can be used as a diagnostic/therapeutic biomarker, we analyzed HTR2A promoter DNA methylation in DNA extracted from the saliva of patients with SCZ and BD, and their first degree relatives versus normal controls. Bisulfite sequencing was used to screen DNA methylation status of the HTR2A promoter CpGs and qMSP was used to quantify the degree of cytosine methylation at differentially methylated sites. Most of the cytosines of the HTR2A promoter were unmethylated. However, CpGs of the -1438A/G polymorphism site, -1420 and -1223 were >95% methylated. The CpG at T102C polymorphic site and neighboring CpGs were ∼70% methylated both in the patients and controls. qMSP analysis revealed that the cytosine of the T102C polymorphic site was significantly hypo-methylated in SCZ, BD, and their first degree relatives compared to the controls. Cytosine methylation of HTR2A at T102C polymorphic site in DNA derived from the saliva can potentially be used as a diagnostic, prognostic, and/or therapeutic biomarker in SCZ and BD. However, these preliminary observations need to be replicated in other populations with a larger sample size to be considered for clinical applications. © 2011 Wiley-Liss, Inc.	topic_bd
77731	10	356219	7	NULL	NULL	NULL	NULL	HTR2A	GP	cytosine of	hypo-methylated in				T102C polymorphic site	SCZ	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Several lines of evidence indicate that dysfunction of serotonin signaling and HTR2A receptor are involved in the pathogenesis of schizophrenia (SCZ) and bipolar disorder (BD). DNA methylation of HTR2A at T102C polymorphic site influences HTR2A expression and aberrant DNA methylation of HTR2A promoter was reported in postmortem brain of patients with SCZ and BD. Hypothesizing that the brain's epigenetic alteration of HTR2A may also exist in peripheral tissues that can be used as a diagnostic/therapeutic biomarker, we analyzed HTR2A promoter DNA methylation in DNA extracted from the saliva of patients with SCZ and BD, and their first degree relatives versus normal controls. Bisulfite sequencing was used to screen DNA methylation status of the HTR2A promoter CpGs and qMSP was used to quantify the degree of cytosine methylation at differentially methylated sites. Most of the cytosines of the HTR2A promoter were unmethylated. However, CpGs of the -1438A/G polymorphism site, -1420 and -1223 were >95% methylated. The CpG at T102C polymorphic site and neighboring CpGs were ∼70% methylated both in the patients and controls. qMSP analysis revealed that the cytosine of the T102C polymorphic site was significantly hypo-methylated in SCZ, BD, and their first degree relatives compared to the controls. Cytosine methylation of HTR2A at T102C polymorphic site in DNA derived from the saliva can potentially be used as a diagnostic, prognostic, and/or therapeutic biomarker in SCZ and BD. However, these preliminary observations need to be replicated in other populations with a larger sample size to be considered for clinical applications. © 2011 Wiley-Liss, Inc.	topic_bd
77732	11	356219	7	NULL	NULL	NULL	NULL	HTR2A	GP	cytosine of	hypo-methylated in				T102C polymorphic site	BD	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Several lines of evidence indicate that dysfunction of serotonin signaling and HTR2A receptor are involved in the pathogenesis of schizophrenia (SCZ) and bipolar disorder (BD). DNA methylation of HTR2A at T102C polymorphic site influences HTR2A expression and aberrant DNA methylation of HTR2A promoter was reported in postmortem brain of patients with SCZ and BD. Hypothesizing that the brain's epigenetic alteration of HTR2A may also exist in peripheral tissues that can be used as a diagnostic/therapeutic biomarker, we analyzed HTR2A promoter DNA methylation in DNA extracted from the saliva of patients with SCZ and BD, and their first degree relatives versus normal controls. Bisulfite sequencing was used to screen DNA methylation status of the HTR2A promoter CpGs and qMSP was used to quantify the degree of cytosine methylation at differentially methylated sites. Most of the cytosines of the HTR2A promoter were unmethylated. However, CpGs of the -1438A/G polymorphism site, -1420 and -1223 were >95% methylated. The CpG at T102C polymorphic site and neighboring CpGs were ∼70% methylated both in the patients and controls. qMSP analysis revealed that the cytosine of the T102C polymorphic site was significantly hypo-methylated in SCZ, BD, and their first degree relatives compared to the controls. Cytosine methylation of HTR2A at T102C polymorphic site in DNA derived from the saliva can potentially be used as a diagnostic, prognostic, and/or therapeutic biomarker in SCZ and BD. However, these preliminary observations need to be replicated in other populations with a larger sample size to be considered for clinical applications. © 2011 Wiley-Liss, Inc.	topic_bd
77733	12	356219	7	NULL	NULL	0	NULL	HTR2A	GP	Cytosine methylation of	used as a		potentially		T102C polymorphic site 	SCZ	MedicalFinding	diagnostic marker in			NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence indicate that dysfunction of serotonin signaling and HTR2A receptor are involved in the pathogenesis of schizophrenia (SCZ) and bipolar disorder (BD). DNA methylation of HTR2A at T102C polymorphic site influences HTR2A expression and aberrant DNA methylation of HTR2A promoter was reported in postmortem brain of patients with SCZ and BD. Hypothesizing that the brain's epigenetic alteration of HTR2A may also exist in peripheral tissues that can be used as a diagnostic/therapeutic biomarker, we analyzed HTR2A promoter DNA methylation in DNA extracted from the saliva of patients with SCZ and BD, and their first degree relatives versus normal controls. Bisulfite sequencing was used to screen DNA methylation status of the HTR2A promoter CpGs and qMSP was used to quantify the degree of cytosine methylation at differentially methylated sites. Most of the cytosines of the HTR2A promoter were unmethylated. However, CpGs of the -1438A/G polymorphism site, -1420 and -1223 were >95% methylated. The CpG at T102C polymorphic site and neighboring CpGs were ∼70% methylated both in the patients and controls. qMSP analysis revealed that the cytosine of the T102C polymorphic site was significantly hypo-methylated in SCZ, BD, and their first degree relatives compared to the controls. Cytosine methylation of HTR2A at T102C polymorphic site in DNA derived from the saliva can potentially be used as a diagnostic, prognostic, and/or therapeutic biomarker in SCZ and BD. However, these preliminary observations need to be replicated in other populations with a larger sample size to be considered for clinical applications. © 2011 Wiley-Liss, Inc.	topic_bd
77734	13	356219	7	NULL	NULL	NULL	NULL	HTR2A	GP	Cytosine methylation of	used as a 		potentially		T102C polymorphic site	SCZ	MedicalFinding	prognostic marker in			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Several lines of evidence indicate that dysfunction of serotonin signaling and HTR2A receptor are involved in the pathogenesis of schizophrenia (SCZ) and bipolar disorder (BD). DNA methylation of HTR2A at T102C polymorphic site influences HTR2A expression and aberrant DNA methylation of HTR2A promoter was reported in postmortem brain of patients with SCZ and BD. Hypothesizing that the brain's epigenetic alteration of HTR2A may also exist in peripheral tissues that can be used as a diagnostic/therapeutic biomarker, we analyzed HTR2A promoter DNA methylation in DNA extracted from the saliva of patients with SCZ and BD, and their first degree relatives versus normal controls. Bisulfite sequencing was used to screen DNA methylation status of the HTR2A promoter CpGs and qMSP was used to quantify the degree of cytosine methylation at differentially methylated sites. Most of the cytosines of the HTR2A promoter were unmethylated. However, CpGs of the -1438A/G polymorphism site, -1420 and -1223 were >95% methylated. The CpG at T102C polymorphic site and neighboring CpGs were ∼70% methylated both in the patients and controls. qMSP analysis revealed that the cytosine of the T102C polymorphic site was significantly hypo-methylated in SCZ, BD, and their first degree relatives compared to the controls. Cytosine methylation of HTR2A at T102C polymorphic site in DNA derived from the saliva can potentially be used as a diagnostic, prognostic, and/or therapeutic biomarker in SCZ and BD. However, these preliminary observations need to be replicated in other populations with a larger sample size to be considered for clinical applications. © 2011 Wiley-Liss, Inc.	topic_bd
77762	14	356219	7	NULL	NULL	0	NULL	HTR2A	GP	Cytosine methylation of	used as a		potentially		T102C polymorphic site	SCZ	MedicalFinding	therapeutic biomarker in			NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence indicate that dysfunction of serotonin signaling and HTR2A receptor are involved in the pathogenesis of schizophrenia (SCZ) and bipolar disorder (BD). DNA methylation of HTR2A at T102C polymorphic site influences HTR2A expression and aberrant DNA methylation of HTR2A promoter was reported in postmortem brain of patients with SCZ and BD. Hypothesizing that the brain's epigenetic alteration of HTR2A may also exist in peripheral tissues that can be used as a diagnostic/therapeutic biomarker, we analyzed HTR2A promoter DNA methylation in DNA extracted from the saliva of patients with SCZ and BD, and their first degree relatives versus normal controls. Bisulfite sequencing was used to screen DNA methylation status of the HTR2A promoter CpGs and qMSP was used to quantify the degree of cytosine methylation at differentially methylated sites. Most of the cytosines of the HTR2A promoter were unmethylated. However, CpGs of the -1438A/G polymorphism site, -1420 and -1223 were >95% methylated. The CpG at T102C polymorphic site and neighboring CpGs were ∼70% methylated both in the patients and controls. qMSP analysis revealed that the cytosine of the T102C polymorphic site was significantly hypo-methylated in SCZ, BD, and their first degree relatives compared to the controls. Cytosine methylation of HTR2A at T102C polymorphic site in DNA derived from the saliva can potentially be used as a diagnostic, prognostic, and/or therapeutic biomarker in SCZ and BD. However, these preliminary observations need to be replicated in other populations with a larger sample size to be considered for clinical applications. © 2011 Wiley-Liss, Inc.	topic_bd
77763	15	356219	7	NULL	NULL	NULL	NULL	HTR2A	GP	Cytosine methylation of	used as a		potentially		T102C polymorphic site	BD	MedicalFinding	diagnostic marker in			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Several lines of evidence indicate that dysfunction of serotonin signaling and HTR2A receptor are involved in the pathogenesis of schizophrenia (SCZ) and bipolar disorder (BD). DNA methylation of HTR2A at T102C polymorphic site influences HTR2A expression and aberrant DNA methylation of HTR2A promoter was reported in postmortem brain of patients with SCZ and BD. Hypothesizing that the brain's epigenetic alteration of HTR2A may also exist in peripheral tissues that can be used as a diagnostic/therapeutic biomarker, we analyzed HTR2A promoter DNA methylation in DNA extracted from the saliva of patients with SCZ and BD, and their first degree relatives versus normal controls. Bisulfite sequencing was used to screen DNA methylation status of the HTR2A promoter CpGs and qMSP was used to quantify the degree of cytosine methylation at differentially methylated sites. Most of the cytosines of the HTR2A promoter were unmethylated. However, CpGs of the -1438A/G polymorphism site, -1420 and -1223 were >95% methylated. The CpG at T102C polymorphic site and neighboring CpGs were ∼70% methylated both in the patients and controls. qMSP analysis revealed that the cytosine of the T102C polymorphic site was significantly hypo-methylated in SCZ, BD, and their first degree relatives compared to the controls. Cytosine methylation of HTR2A at T102C polymorphic site in DNA derived from the saliva can potentially be used as a diagnostic, prognostic, and/or therapeutic biomarker in SCZ and BD. However, these preliminary observations need to be replicated in other populations with a larger sample size to be considered for clinical applications. © 2011 Wiley-Liss, Inc.	topic_bd
77764	16	356219	7	NULL	NULL	NULL	NULL	HTR2A	GP	Cytosine methylation of	used as a		potentially		T102C polymorphic site	BD	MedicalFinding	prognostic marker in			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Several lines of evidence indicate that dysfunction of serotonin signaling and HTR2A receptor are involved in the pathogenesis of schizophrenia (SCZ) and bipolar disorder (BD). DNA methylation of HTR2A at T102C polymorphic site influences HTR2A expression and aberrant DNA methylation of HTR2A promoter was reported in postmortem brain of patients with SCZ and BD. Hypothesizing that the brain's epigenetic alteration of HTR2A may also exist in peripheral tissues that can be used as a diagnostic/therapeutic biomarker, we analyzed HTR2A promoter DNA methylation in DNA extracted from the saliva of patients with SCZ and BD, and their first degree relatives versus normal controls. Bisulfite sequencing was used to screen DNA methylation status of the HTR2A promoter CpGs and qMSP was used to quantify the degree of cytosine methylation at differentially methylated sites. Most of the cytosines of the HTR2A promoter were unmethylated. However, CpGs of the -1438A/G polymorphism site, -1420 and -1223 were >95% methylated. The CpG at T102C polymorphic site and neighboring CpGs were ∼70% methylated both in the patients and controls. qMSP analysis revealed that the cytosine of the T102C polymorphic site was significantly hypo-methylated in SCZ, BD, and their first degree relatives compared to the controls. Cytosine methylation of HTR2A at T102C polymorphic site in DNA derived from the saliva can potentially be used as a diagnostic, prognostic, and/or therapeutic biomarker in SCZ and BD. However, these preliminary observations need to be replicated in other populations with a larger sample size to be considered for clinical applications. © 2011 Wiley-Liss, Inc.	topic_bd
77765	17	356219	7	NULL	NULL	0	NULL	HTR2A	GP	Cytosine methylation of	used as a		potentially		T102C polymorphic site	BD	MedicalFinding	therapeutic biomarker in			NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence indicate that dysfunction of serotonin signaling and HTR2A receptor are involved in the pathogenesis of schizophrenia (SCZ) and bipolar disorder (BD). DNA methylation of HTR2A at T102C polymorphic site influences HTR2A expression and aberrant DNA methylation of HTR2A promoter was reported in postmortem brain of patients with SCZ and BD. Hypothesizing that the brain's epigenetic alteration of HTR2A may also exist in peripheral tissues that can be used as a diagnostic/therapeutic biomarker, we analyzed HTR2A promoter DNA methylation in DNA extracted from the saliva of patients with SCZ and BD, and their first degree relatives versus normal controls. Bisulfite sequencing was used to screen DNA methylation status of the HTR2A promoter CpGs and qMSP was used to quantify the degree of cytosine methylation at differentially methylated sites. Most of the cytosines of the HTR2A promoter were unmethylated. However, CpGs of the -1438A/G polymorphism site, -1420 and -1223 were >95% methylated. The CpG at T102C polymorphic site and neighboring CpGs were ∼70% methylated both in the patients and controls. qMSP analysis revealed that the cytosine of the T102C polymorphic site was significantly hypo-methylated in SCZ, BD, and their first degree relatives compared to the controls. Cytosine methylation of HTR2A at T102C polymorphic site in DNA derived from the saliva can potentially be used as a diagnostic, prognostic, and/or therapeutic biomarker in SCZ and BD. However, these preliminary observations need to be replicated in other populations with a larger sample size to be considered for clinical applications. © 2011 Wiley-Liss, Inc.	topic_bd
77767	18	356219	7	NULL	NULL	0	NULL	SCZ	MedicalFinding		is					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence indicate that dysfunction of serotonin signaling and HTR2A receptor are involved in the pathogenesis of schizophrenia (SCZ) and bipolar disorder (BD). DNA methylation of HTR2A at T102C polymorphic site influences HTR2A expression and aberrant DNA methylation of HTR2A promoter was reported in postmortem brain of patients with SCZ and BD. Hypothesizing that the brain's epigenetic alteration of HTR2A may also exist in peripheral tissues that can be used as a diagnostic/therapeutic biomarker, we analyzed HTR2A promoter DNA methylation in DNA extracted from the saliva of patients with SCZ and BD, and their first degree relatives versus normal controls. Bisulfite sequencing was used to screen DNA methylation status of the HTR2A promoter CpGs and qMSP was used to quantify the degree of cytosine methylation at differentially methylated sites. Most of the cytosines of the HTR2A promoter were unmethylated. However, CpGs of the -1438A/G polymorphism site, -1420 and -1223 were >95% methylated. The CpG at T102C polymorphic site and neighboring CpGs were ∼70% methylated both in the patients and controls. qMSP analysis revealed that the cytosine of the T102C polymorphic site was significantly hypo-methylated in SCZ, BD, and their first degree relatives compared to the controls. Cytosine methylation of HTR2A at T102C polymorphic site in DNA derived from the saliva can potentially be used as a diagnostic, prognostic, and/or therapeutic biomarker in SCZ and BD. However, these preliminary observations need to be replicated in other populations with a larger sample size to be considered for clinical applications. © 2011 Wiley-Liss, Inc.	topic_bd
77768	19	356219	7	NULL	NULL	0	NULL	BD	MedicalFinding		is					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence indicate that dysfunction of serotonin signaling and HTR2A receptor are involved in the pathogenesis of schizophrenia (SCZ) and bipolar disorder (BD). DNA methylation of HTR2A at T102C polymorphic site influences HTR2A expression and aberrant DNA methylation of HTR2A promoter was reported in postmortem brain of patients with SCZ and BD. Hypothesizing that the brain's epigenetic alteration of HTR2A may also exist in peripheral tissues that can be used as a diagnostic/therapeutic biomarker, we analyzed HTR2A promoter DNA methylation in DNA extracted from the saliva of patients with SCZ and BD, and their first degree relatives versus normal controls. Bisulfite sequencing was used to screen DNA methylation status of the HTR2A promoter CpGs and qMSP was used to quantify the degree of cytosine methylation at differentially methylated sites. Most of the cytosines of the HTR2A promoter were unmethylated. However, CpGs of the -1438A/G polymorphism site, -1420 and -1223 were >95% methylated. The CpG at T102C polymorphic site and neighboring CpGs were ∼70% methylated both in the patients and controls. qMSP analysis revealed that the cytosine of the T102C polymorphic site was significantly hypo-methylated in SCZ, BD, and their first degree relatives compared to the controls. Cytosine methylation of HTR2A at T102C polymorphic site in DNA derived from the saliva can potentially be used as a diagnostic, prognostic, and/or therapeutic biomarker in SCZ and BD. However, these preliminary observations need to be replicated in other populations with a larger sample size to be considered for clinical applications. © 2011 Wiley-Liss, Inc.	topic_bd
77766	1	356220	7	NULL	NULL	0	NULL	HPA axis	OrganismPart		dysregulated in					BD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract INTRODUCTION: The hypothalamus-pituitary-adrenal (HPA)-axis is often found to be dysregulated in bipolar disorder (BD) while stress and changes in day-night rhythms can trigger a new mood episode. Genetic variants of the glucocorticoid receptor (GR)- and mineralocorticoid receptor (MR)-gene influence both the reactivity of the stress-response and associate with changes in mood. In this study we tested the hypothesis that these polymorphisms associate with different clinical characteristics of BD. METHODS: We studied 326 outpatients with BD and performed GR genotyping of the TthIIII, ER22/23EK, N363S, BclI, and 9β polymorphisms, as well as MR genotyping of the 2G/C and I180V variants. All patients were interviewed for clinical characteristics. RESULTS: Seasonal patterns of hypomania are related to the BclI haplotype and the TthIIII+9β haplotype of the GR gene (respectively, crude p=.007 and crude p=.005). Carriers of the ER22/23EK polymorphism had an almost 8 years earlier onset of their first (hypo)manic episode than non-carriers (crude p=.004, after adjustment p=.016). No evidence for a role of the MR in modifying clinical manifestations was found. CONCLUSION: Polymorphisms of the GR-gene are factors which influence some clinical manifestations of BD, with respect to seasonal pattern of (hypo)mania and age of onset.	topic_bd
77769	2	356220	7	NULL	NULL	0	NULL	stress	MentalProcess		triggers					new mood episode	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract INTRODUCTION: The hypothalamus-pituitary-adrenal (HPA)-axis is often found to be dysregulated in bipolar disorder (BD) while stress and changes in day-night rhythms can trigger a new mood episode. Genetic variants of the glucocorticoid receptor (GR)- and mineralocorticoid receptor (MR)-gene influence both the reactivity of the stress-response and associate with changes in mood. In this study we tested the hypothesis that these polymorphisms associate with different clinical characteristics of BD. METHODS: We studied 326 outpatients with BD and performed GR genotyping of the TthIIII, ER22/23EK, N363S, BclI, and 9β polymorphisms, as well as MR genotyping of the 2G/C and I180V variants. All patients were interviewed for clinical characteristics. RESULTS: Seasonal patterns of hypomania are related to the BclI haplotype and the TthIIII+9β haplotype of the GR gene (respectively, crude p=.007 and crude p=.005). Carriers of the ER22/23EK polymorphism had an almost 8 years earlier onset of their first (hypo)manic episode than non-carriers (crude p=.004, after adjustment p=.016). No evidence for a role of the MR in modifying clinical manifestations was found. CONCLUSION: Polymorphisms of the GR-gene are factors which influence some clinical manifestations of BD, with respect to seasonal pattern of (hypo)mania and age of onset.	topic_bd
77770	3	356220	7	NULL	NULL	0	NULL	day-night rhythms	MentalProcess		trigger					new mood episode	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract INTRODUCTION: The hypothalamus-pituitary-adrenal (HPA)-axis is often found to be dysregulated in bipolar disorder (BD) while stress and changes in day-night rhythms can trigger a new mood episode. Genetic variants of the glucocorticoid receptor (GR)- and mineralocorticoid receptor (MR)-gene influence both the reactivity of the stress-response and associate with changes in mood. In this study we tested the hypothesis that these polymorphisms associate with different clinical characteristics of BD. METHODS: We studied 326 outpatients with BD and performed GR genotyping of the TthIIII, ER22/23EK, N363S, BclI, and 9β polymorphisms, as well as MR genotyping of the 2G/C and I180V variants. All patients were interviewed for clinical characteristics. RESULTS: Seasonal patterns of hypomania are related to the BclI haplotype and the TthIIII+9β haplotype of the GR gene (respectively, crude p=.007 and crude p=.005). Carriers of the ER22/23EK polymorphism had an almost 8 years earlier onset of their first (hypo)manic episode than non-carriers (crude p=.004, after adjustment p=.016). No evidence for a role of the MR in modifying clinical manifestations was found. CONCLUSION: Polymorphisms of the GR-gene are factors which influence some clinical manifestations of BD, with respect to seasonal pattern of (hypo)mania and age of onset.	topic_bd
77771	4	356220	7	NULL	NULL	0	NULL	GR gene	GP	genetic variants of	influence					stress-response	MentalProcess	reactivity of			NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract INTRODUCTION: The hypothalamus-pituitary-adrenal (HPA)-axis is often found to be dysregulated in bipolar disorder (BD) while stress and changes in day-night rhythms can trigger a new mood episode. Genetic variants of the glucocorticoid receptor (GR)- and mineralocorticoid receptor (MR)-gene influence both the reactivity of the stress-response and associate with changes in mood. In this study we tested the hypothesis that these polymorphisms associate with different clinical characteristics of BD. METHODS: We studied 326 outpatients with BD and performed GR genotyping of the TthIIII, ER22/23EK, N363S, BclI, and 9β polymorphisms, as well as MR genotyping of the 2G/C and I180V variants. All patients were interviewed for clinical characteristics. RESULTS: Seasonal patterns of hypomania are related to the BclI haplotype and the TthIIII+9β haplotype of the GR gene (respectively, crude p=.007 and crude p=.005). Carriers of the ER22/23EK polymorphism had an almost 8 years earlier onset of their first (hypo)manic episode than non-carriers (crude p=.004, after adjustment p=.016). No evidence for a role of the MR in modifying clinical manifestations was found. CONCLUSION: Polymorphisms of the GR-gene are factors which influence some clinical manifestations of BD, with respect to seasonal pattern of (hypo)mania and age of onset.	topic_bd
77772	5	356220	7	NULL	NULL	0	NULL	MR gene	GP	genetic variants of	influence					stress-response	MentalProcess	reactivity of			NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract INTRODUCTION: The hypothalamus-pituitary-adrenal (HPA)-axis is often found to be dysregulated in bipolar disorder (BD) while stress and changes in day-night rhythms can trigger a new mood episode. Genetic variants of the glucocorticoid receptor (GR)- and mineralocorticoid receptor (MR)-gene influence both the reactivity of the stress-response and associate with changes in mood. In this study we tested the hypothesis that these polymorphisms associate with different clinical characteristics of BD. METHODS: We studied 326 outpatients with BD and performed GR genotyping of the TthIIII, ER22/23EK, N363S, BclI, and 9β polymorphisms, as well as MR genotyping of the 2G/C and I180V variants. All patients were interviewed for clinical characteristics. RESULTS: Seasonal patterns of hypomania are related to the BclI haplotype and the TthIIII+9β haplotype of the GR gene (respectively, crude p=.007 and crude p=.005). Carriers of the ER22/23EK polymorphism had an almost 8 years earlier onset of their first (hypo)manic episode than non-carriers (crude p=.004, after adjustment p=.016). No evidence for a role of the MR in modifying clinical manifestations was found. CONCLUSION: Polymorphisms of the GR-gene are factors which influence some clinical manifestations of BD, with respect to seasonal pattern of (hypo)mania and age of onset.	topic_bd
77773	6	356220	7	NULL	NULL	0	NULL	GR gene	GP	genetic variants of	associate with					mood	MentalProcess	changes in			NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract INTRODUCTION: The hypothalamus-pituitary-adrenal (HPA)-axis is often found to be dysregulated in bipolar disorder (BD) while stress and changes in day-night rhythms can trigger a new mood episode. Genetic variants of the glucocorticoid receptor (GR)- and mineralocorticoid receptor (MR)-gene influence both the reactivity of the stress-response and associate with changes in mood. In this study we tested the hypothesis that these polymorphisms associate with different clinical characteristics of BD. METHODS: We studied 326 outpatients with BD and performed GR genotyping of the TthIIII, ER22/23EK, N363S, BclI, and 9β polymorphisms, as well as MR genotyping of the 2G/C and I180V variants. All patients were interviewed for clinical characteristics. RESULTS: Seasonal patterns of hypomania are related to the BclI haplotype and the TthIIII+9β haplotype of the GR gene (respectively, crude p=.007 and crude p=.005). Carriers of the ER22/23EK polymorphism had an almost 8 years earlier onset of their first (hypo)manic episode than non-carriers (crude p=.004, after adjustment p=.016). No evidence for a role of the MR in modifying clinical manifestations was found. CONCLUSION: Polymorphisms of the GR-gene are factors which influence some clinical manifestations of BD, with respect to seasonal pattern of (hypo)mania and age of onset.	topic_bd
77774	7	356220	7	NULL	NULL	0	NULL	MR gene	GP	genetic variants of	associate with					mood	MentalProcess	changes in			NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract INTRODUCTION: The hypothalamus-pituitary-adrenal (HPA)-axis is often found to be dysregulated in bipolar disorder (BD) while stress and changes in day-night rhythms can trigger a new mood episode. Genetic variants of the glucocorticoid receptor (GR)- and mineralocorticoid receptor (MR)-gene influence both the reactivity of the stress-response and associate with changes in mood. In this study we tested the hypothesis that these polymorphisms associate with different clinical characteristics of BD. METHODS: We studied 326 outpatients with BD and performed GR genotyping of the TthIIII, ER22/23EK, N363S, BclI, and 9β polymorphisms, as well as MR genotyping of the 2G/C and I180V variants. All patients were interviewed for clinical characteristics. RESULTS: Seasonal patterns of hypomania are related to the BclI haplotype and the TthIIII+9β haplotype of the GR gene (respectively, crude p=.007 and crude p=.005). Carriers of the ER22/23EK polymorphism had an almost 8 years earlier onset of their first (hypo)manic episode than non-carriers (crude p=.004, after adjustment p=.016). No evidence for a role of the MR in modifying clinical manifestations was found. CONCLUSION: Polymorphisms of the GR-gene are factors which influence some clinical manifestations of BD, with respect to seasonal pattern of (hypo)mania and age of onset.	topic_bd
77775	8	356220	7	NULL	NULL	0	NULL	GR-gene	GP	Polymorphisms of	influence					BD	MedicalFinding	clinical manifestations of 			NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract INTRODUCTION: The hypothalamus-pituitary-adrenal (HPA)-axis is often found to be dysregulated in bipolar disorder (BD) while stress and changes in day-night rhythms can trigger a new mood episode. Genetic variants of the glucocorticoid receptor (GR)- and mineralocorticoid receptor (MR)-gene influence both the reactivity of the stress-response and associate with changes in mood. In this study we tested the hypothesis that these polymorphisms associate with different clinical characteristics of BD. METHODS: We studied 326 outpatients with BD and performed GR genotyping of the TthIIII, ER22/23EK, N363S, BclI, and 9β polymorphisms, as well as MR genotyping of the 2G/C and I180V variants. All patients were interviewed for clinical characteristics. RESULTS: Seasonal patterns of hypomania are related to the BclI haplotype and the TthIIII+9β haplotype of the GR gene (respectively, crude p=.007 and crude p=.005). Carriers of the ER22/23EK polymorphism had an almost 8 years earlier onset of their first (hypo)manic episode than non-carriers (crude p=.004, after adjustment p=.016). No evidence for a role of the MR in modifying clinical manifestations was found. CONCLUSION: Polymorphisms of the GR-gene are factors which influence some clinical manifestations of BD, with respect to seasonal pattern of (hypo)mania and age of onset.	topic_bd
77776	9	356220	7	NULL	NULL	0	NULL	HPA axis	OrganismPart		is					hypothalamus-pituitary-adrenal -axis					NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract INTRODUCTION: The hypothalamus-pituitary-adrenal (HPA)-axis is often found to be dysregulated in bipolar disorder (BD) while stress and changes in day-night rhythms can trigger a new mood episode. Genetic variants of the glucocorticoid receptor (GR)- and mineralocorticoid receptor (MR)-gene influence both the reactivity of the stress-response and associate with changes in mood. In this study we tested the hypothesis that these polymorphisms associate with different clinical characteristics of BD. METHODS: We studied 326 outpatients with BD and performed GR genotyping of the TthIIII, ER22/23EK, N363S, BclI, and 9β polymorphisms, as well as MR genotyping of the 2G/C and I180V variants. All patients were interviewed for clinical characteristics. RESULTS: Seasonal patterns of hypomania are related to the BclI haplotype and the TthIIII+9β haplotype of the GR gene (respectively, crude p=.007 and crude p=.005). Carriers of the ER22/23EK polymorphism had an almost 8 years earlier onset of their first (hypo)manic episode than non-carriers (crude p=.004, after adjustment p=.016). No evidence for a role of the MR in modifying clinical manifestations was found. CONCLUSION: Polymorphisms of the GR-gene are factors which influence some clinical manifestations of BD, with respect to seasonal pattern of (hypo)mania and age of onset.	topic_bd
77777	10	356220	7	NULL	NULL	0	NULL	GR	GP		is					glucocorticoid receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract INTRODUCTION: The hypothalamus-pituitary-adrenal (HPA)-axis is often found to be dysregulated in bipolar disorder (BD) while stress and changes in day-night rhythms can trigger a new mood episode. Genetic variants of the glucocorticoid receptor (GR)- and mineralocorticoid receptor (MR)-gene influence both the reactivity of the stress-response and associate with changes in mood. In this study we tested the hypothesis that these polymorphisms associate with different clinical characteristics of BD. METHODS: We studied 326 outpatients with BD and performed GR genotyping of the TthIIII, ER22/23EK, N363S, BclI, and 9β polymorphisms, as well as MR genotyping of the 2G/C and I180V variants. All patients were interviewed for clinical characteristics. RESULTS: Seasonal patterns of hypomania are related to the BclI haplotype and the TthIIII+9β haplotype of the GR gene (respectively, crude p=.007 and crude p=.005). Carriers of the ER22/23EK polymorphism had an almost 8 years earlier onset of their first (hypo)manic episode than non-carriers (crude p=.004, after adjustment p=.016). No evidence for a role of the MR in modifying clinical manifestations was found. CONCLUSION: Polymorphisms of the GR-gene are factors which influence some clinical manifestations of BD, with respect to seasonal pattern of (hypo)mania and age of onset.	topic_bd
77778	11	356220	7	NULL	NULL	0	NULL	MR	GP		is					mineralocorticoid receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract INTRODUCTION: The hypothalamus-pituitary-adrenal (HPA)-axis is often found to be dysregulated in bipolar disorder (BD) while stress and changes in day-night rhythms can trigger a new mood episode. Genetic variants of the glucocorticoid receptor (GR)- and mineralocorticoid receptor (MR)-gene influence both the reactivity of the stress-response and associate with changes in mood. In this study we tested the hypothesis that these polymorphisms associate with different clinical characteristics of BD. METHODS: We studied 326 outpatients with BD and performed GR genotyping of the TthIIII, ER22/23EK, N363S, BclI, and 9β polymorphisms, as well as MR genotyping of the 2G/C and I180V variants. All patients were interviewed for clinical characteristics. RESULTS: Seasonal patterns of hypomania are related to the BclI haplotype and the TthIIII+9β haplotype of the GR gene (respectively, crude p=.007 and crude p=.005). Carriers of the ER22/23EK polymorphism had an almost 8 years earlier onset of their first (hypo)manic episode than non-carriers (crude p=.004, after adjustment p=.016). No evidence for a role of the MR in modifying clinical manifestations was found. CONCLUSION: Polymorphisms of the GR-gene are factors which influence some clinical manifestations of BD, with respect to seasonal pattern of (hypo)mania and age of onset.	topic_bd
77781	12	356220	7	NULL	NULL	0	NULL	BD	MedicalFinding		is					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract INTRODUCTION: The hypothalamus-pituitary-adrenal (HPA)-axis is often found to be dysregulated in bipolar disorder (BD) while stress and changes in day-night rhythms can trigger a new mood episode. Genetic variants of the glucocorticoid receptor (GR)- and mineralocorticoid receptor (MR)-gene influence both the reactivity of the stress-response and associate with changes in mood. In this study we tested the hypothesis that these polymorphisms associate with different clinical characteristics of BD. METHODS: We studied 326 outpatients with BD and performed GR genotyping of the TthIIII, ER22/23EK, N363S, BclI, and 9β polymorphisms, as well as MR genotyping of the 2G/C and I180V variants. All patients were interviewed for clinical characteristics. RESULTS: Seasonal patterns of hypomania are related to the BclI haplotype and the TthIIII+9β haplotype of the GR gene (respectively, crude p=.007 and crude p=.005). Carriers of the ER22/23EK polymorphism had an almost 8 years earlier onset of their first (hypo)manic episode than non-carriers (crude p=.004, after adjustment p=.016). No evidence for a role of the MR in modifying clinical manifestations was found. CONCLUSION: Polymorphisms of the GR-gene are factors which influence some clinical manifestations of BD, with respect to seasonal pattern of (hypo)mania and age of onset.	topic_bd
77779	1	356222	7	NULL	NULL	0	NULL	Psychotic features	MedicalFinding		defined as					delusions	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Psychotic features, defined as delusions or hallucinations, commonly occur in bipolar disorder (BP) and may be indicative of a more homogeneous form of the illness, with possible etiologic ties to schizophrenia. Several studies have shown that psychotic features aggregate in bipolar families, and increased interest in the molecular genetics of psychotic BP is emerging. Although preliminary, linkage studies of psychotic BP show replicated evidence for suggestive genome-wide linkage to chromosomes 8p and 13q, which have been implicated in prior linkage studies of schizophrenia and BP. Association studies of psychotic BP and subtypes such as mood-incongruent psychotic BP have uncovered modest positive results for several candidate schizophrenia susceptibility genes, including dysbindin, DAOA/G30, Disrupted-in-Schizophrenia-1, and neuregulin 1. These tentative results are consistent with the hypothesis that the subphenotype of psychotic BP may represent a clinical manifestation of 'overlap' genes between schizophrenia and mood disorder syndromes.	topic_bd
77780	2	356222	7	NULL	NULL	0	NULL	Psychotic features	MedicalFinding		defined as					hallucinations	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Psychotic features, defined as delusions or hallucinations, commonly occur in bipolar disorder (BP) and may be indicative of a more homogeneous form of the illness, with possible etiologic ties to schizophrenia. Several studies have shown that psychotic features aggregate in bipolar families, and increased interest in the molecular genetics of psychotic BP is emerging. Although preliminary, linkage studies of psychotic BP show replicated evidence for suggestive genome-wide linkage to chromosomes 8p and 13q, which have been implicated in prior linkage studies of schizophrenia and BP. Association studies of psychotic BP and subtypes such as mood-incongruent psychotic BP have uncovered modest positive results for several candidate schizophrenia susceptibility genes, including dysbindin, DAOA/G30, Disrupted-in-Schizophrenia-1, and neuregulin 1. These tentative results are consistent with the hypothesis that the subphenotype of psychotic BP may represent a clinical manifestation of 'overlap' genes between schizophrenia and mood disorder syndromes.	topic_bd
78015	3	356222	7	NULL	NULL	0	NULL	statement 1	Process		occur in		commonly			BP	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Psychotic features, defined as delusions or hallucinations, commonly occur in bipolar disorder (BP) and may be indicative of a more homogeneous form of the illness, with possible etiologic ties to schizophrenia. Several studies have shown that psychotic features aggregate in bipolar families, and increased interest in the molecular genetics of psychotic BP is emerging. Although preliminary, linkage studies of psychotic BP show replicated evidence for suggestive genome-wide linkage to chromosomes 8p and 13q, which have been implicated in prior linkage studies of schizophrenia and BP. Association studies of psychotic BP and subtypes such as mood-incongruent psychotic BP have uncovered modest positive results for several candidate schizophrenia susceptibility genes, including dysbindin, DAOA/G30, Disrupted-in-Schizophrenia-1, and neuregulin 1. These tentative results are consistent with the hypothesis that the subphenotype of psychotic BP may represent a clinical manifestation of 'overlap' genes between schizophrenia and mood disorder syndromes.	topic_bd
78016	4	356222	7	NULL	NULL	0	NULL	statement 2	Process		occur in		commonly			BP	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Psychotic features, defined as delusions or hallucinations, commonly occur in bipolar disorder (BP) and may be indicative of a more homogeneous form of the illness, with possible etiologic ties to schizophrenia. Several studies have shown that psychotic features aggregate in bipolar families, and increased interest in the molecular genetics of psychotic BP is emerging. Although preliminary, linkage studies of psychotic BP show replicated evidence for suggestive genome-wide linkage to chromosomes 8p and 13q, which have been implicated in prior linkage studies of schizophrenia and BP. Association studies of psychotic BP and subtypes such as mood-incongruent psychotic BP have uncovered modest positive results for several candidate schizophrenia susceptibility genes, including dysbindin, DAOA/G30, Disrupted-in-Schizophrenia-1, and neuregulin 1. These tentative results are consistent with the hypothesis that the subphenotype of psychotic BP may represent a clinical manifestation of 'overlap' genes between schizophrenia and mood disorder syndromes.	topic_bd
78017	5	356222	7	NULL	NULL	0	NULL	BP	MedicalFinding		is					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Psychotic features, defined as delusions or hallucinations, commonly occur in bipolar disorder (BP) and may be indicative of a more homogeneous form of the illness, with possible etiologic ties to schizophrenia. Several studies have shown that psychotic features aggregate in bipolar families, and increased interest in the molecular genetics of psychotic BP is emerging. Although preliminary, linkage studies of psychotic BP show replicated evidence for suggestive genome-wide linkage to chromosomes 8p and 13q, which have been implicated in prior linkage studies of schizophrenia and BP. Association studies of psychotic BP and subtypes such as mood-incongruent psychotic BP have uncovered modest positive results for several candidate schizophrenia susceptibility genes, including dysbindin, DAOA/G30, Disrupted-in-Schizophrenia-1, and neuregulin 1. These tentative results are consistent with the hypothesis that the subphenotype of psychotic BP may represent a clinical manifestation of 'overlap' genes between schizophrenia and mood disorder syndromes.	topic_bd
78018	6	356222	7	NULL	NULL	0	NULL	statement 3	Process		indicative of					illness	MedicalFinding	homogeneous form of			NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Psychotic features, defined as delusions or hallucinations, commonly occur in bipolar disorder (BP) and may be indicative of a more homogeneous form of the illness, with possible etiologic ties to schizophrenia. Several studies have shown that psychotic features aggregate in bipolar families, and increased interest in the molecular genetics of psychotic BP is emerging. Although preliminary, linkage studies of psychotic BP show replicated evidence for suggestive genome-wide linkage to chromosomes 8p and 13q, which have been implicated in prior linkage studies of schizophrenia and BP. Association studies of psychotic BP and subtypes such as mood-incongruent psychotic BP have uncovered modest positive results for several candidate schizophrenia susceptibility genes, including dysbindin, DAOA/G30, Disrupted-in-Schizophrenia-1, and neuregulin 1. These tentative results are consistent with the hypothesis that the subphenotype of psychotic BP may represent a clinical manifestation of 'overlap' genes between schizophrenia and mood disorder syndromes.	topic_bd
78019	7	356222	7	NULL	NULL	0	NULL	statement 4	Process		indicative of					illness	MedicalFinding	homogeneous form of			NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Psychotic features, defined as delusions or hallucinations, commonly occur in bipolar disorder (BP) and may be indicative of a more homogeneous form of the illness, with possible etiologic ties to schizophrenia. Several studies have shown that psychotic features aggregate in bipolar families, and increased interest in the molecular genetics of psychotic BP is emerging. Although preliminary, linkage studies of psychotic BP show replicated evidence for suggestive genome-wide linkage to chromosomes 8p and 13q, which have been implicated in prior linkage studies of schizophrenia and BP. Association studies of psychotic BP and subtypes such as mood-incongruent psychotic BP have uncovered modest positive results for several candidate schizophrenia susceptibility genes, including dysbindin, DAOA/G30, Disrupted-in-Schizophrenia-1, and neuregulin 1. These tentative results are consistent with the hypothesis that the subphenotype of psychotic BP may represent a clinical manifestation of 'overlap' genes between schizophrenia and mood disorder syndromes.	topic_bd
78020	8	356222	7	NULL	NULL	0	NULL	statement 3	Process		etiologic ties to		possible			schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Psychotic features, defined as delusions or hallucinations, commonly occur in bipolar disorder (BP) and may be indicative of a more homogeneous form of the illness, with possible etiologic ties to schizophrenia. Several studies have shown that psychotic features aggregate in bipolar families, and increased interest in the molecular genetics of psychotic BP is emerging. Although preliminary, linkage studies of psychotic BP show replicated evidence for suggestive genome-wide linkage to chromosomes 8p and 13q, which have been implicated in prior linkage studies of schizophrenia and BP. Association studies of psychotic BP and subtypes such as mood-incongruent psychotic BP have uncovered modest positive results for several candidate schizophrenia susceptibility genes, including dysbindin, DAOA/G30, Disrupted-in-Schizophrenia-1, and neuregulin 1. These tentative results are consistent with the hypothesis that the subphenotype of psychotic BP may represent a clinical manifestation of 'overlap' genes between schizophrenia and mood disorder syndromes.	topic_bd
78021	9	356222	7	NULL	NULL	0	NULL	statement 4	Process		etiologic ties to		possible			schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Psychotic features, defined as delusions or hallucinations, commonly occur in bipolar disorder (BP) and may be indicative of a more homogeneous form of the illness, with possible etiologic ties to schizophrenia. Several studies have shown that psychotic features aggregate in bipolar families, and increased interest in the molecular genetics of psychotic BP is emerging. Although preliminary, linkage studies of psychotic BP show replicated evidence for suggestive genome-wide linkage to chromosomes 8p and 13q, which have been implicated in prior linkage studies of schizophrenia and BP. Association studies of psychotic BP and subtypes such as mood-incongruent psychotic BP have uncovered modest positive results for several candidate schizophrenia susceptibility genes, including dysbindin, DAOA/G30, Disrupted-in-Schizophrenia-1, and neuregulin 1. These tentative results are consistent with the hypothesis that the subphenotype of psychotic BP may represent a clinical manifestation of 'overlap' genes between schizophrenia and mood disorder syndromes.	topic_bd
78022	10	356222	7	NULL	NULL	NULL	NULL	psychotic BP	MedicalFinding		show					chromosome 8p	Chromosome	evidence for suggestive genome-wide linkage to			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Abstract Psychotic features, defined as delusions or hallucinations, commonly occur in bipolar disorder (BP) and may be indicative of a more homogeneous form of the illness, with possible etiologic ties to schizophrenia. Several studies have shown that psychotic features aggregate in bipolar families, and increased interest in the molecular genetics of psychotic BP is emerging. Although preliminary, linkage studies of psychotic BP show replicated evidence for suggestive genome-wide linkage to chromosomes 8p and 13q, which have been implicated in prior linkage studies of schizophrenia and BP. Association studies of psychotic BP and subtypes such as mood-incongruent psychotic BP have uncovered modest positive results for several candidate schizophrenia susceptibility genes, including dysbindin, DAOA/G30, Disrupted-in-Schizophrenia-1, and neuregulin 1. These tentative results are consistent with the hypothesis that the subphenotype of psychotic BP may represent a clinical manifestation of 'overlap' genes between schizophrenia and mood disorder syndromes.	topic_bd
78023	11	356222	7	NULL	NULL	NULL	NULL	psychotic BP	MedicalFinding		show					chromosome 13q	Chromosome	evidence for suggestive genome-wide linkage to			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Abstract Psychotic features, defined as delusions or hallucinations, commonly occur in bipolar disorder (BP) and may be indicative of a more homogeneous form of the illness, with possible etiologic ties to schizophrenia. Several studies have shown that psychotic features aggregate in bipolar families, and increased interest in the molecular genetics of psychotic BP is emerging. Although preliminary, linkage studies of psychotic BP show replicated evidence for suggestive genome-wide linkage to chromosomes 8p and 13q, which have been implicated in prior linkage studies of schizophrenia and BP. Association studies of psychotic BP and subtypes such as mood-incongruent psychotic BP have uncovered modest positive results for several candidate schizophrenia susceptibility genes, including dysbindin, DAOA/G30, Disrupted-in-Schizophrenia-1, and neuregulin 1. These tentative results are consistent with the hypothesis that the subphenotype of psychotic BP may represent a clinical manifestation of 'overlap' genes between schizophrenia and mood disorder syndromes.	topic_bd
78024	12	356222	7	NULL	NULL	0	NULL	dysbindin	GP		is a type of					schizophrenia susceptibility genes	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Psychotic features, defined as delusions or hallucinations, commonly occur in bipolar disorder (BP) and may be indicative of a more homogeneous form of the illness, with possible etiologic ties to schizophrenia. Several studies have shown that psychotic features aggregate in bipolar families, and increased interest in the molecular genetics of psychotic BP is emerging. Although preliminary, linkage studies of psychotic BP show replicated evidence for suggestive genome-wide linkage to chromosomes 8p and 13q, which have been implicated in prior linkage studies of schizophrenia and BP. Association studies of psychotic BP and subtypes such as mood-incongruent psychotic BP have uncovered modest positive results for several candidate schizophrenia susceptibility genes, including dysbindin, DAOA/G30, Disrupted-in-Schizophrenia-1, and neuregulin 1. These tentative results are consistent with the hypothesis that the subphenotype of psychotic BP may represent a clinical manifestation of 'overlap' genes between schizophrenia and mood disorder syndromes.	topic_bd
78025	13	356222	7	NULL	NULL	0	NULL	DAOA/G30	GP		is a type of					schizophrenia susceptibility genes	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Psychotic features, defined as delusions or hallucinations, commonly occur in bipolar disorder (BP) and may be indicative of a more homogeneous form of the illness, with possible etiologic ties to schizophrenia. Several studies have shown that psychotic features aggregate in bipolar families, and increased interest in the molecular genetics of psychotic BP is emerging. Although preliminary, linkage studies of psychotic BP show replicated evidence for suggestive genome-wide linkage to chromosomes 8p and 13q, which have been implicated in prior linkage studies of schizophrenia and BP. Association studies of psychotic BP and subtypes such as mood-incongruent psychotic BP have uncovered modest positive results for several candidate schizophrenia susceptibility genes, including dysbindin, DAOA/G30, Disrupted-in-Schizophrenia-1, and neuregulin 1. These tentative results are consistent with the hypothesis that the subphenotype of psychotic BP may represent a clinical manifestation of 'overlap' genes between schizophrenia and mood disorder syndromes.	topic_bd
78026	14	356222	7	NULL	NULL	0	NULL	Disrupted-in-Schizophrenia-1	GP		is a type of					schizophrenia susceptibility genes	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Psychotic features, defined as delusions or hallucinations, commonly occur in bipolar disorder (BP) and may be indicative of a more homogeneous form of the illness, with possible etiologic ties to schizophrenia. Several studies have shown that psychotic features aggregate in bipolar families, and increased interest in the molecular genetics of psychotic BP is emerging. Although preliminary, linkage studies of psychotic BP show replicated evidence for suggestive genome-wide linkage to chromosomes 8p and 13q, which have been implicated in prior linkage studies of schizophrenia and BP. Association studies of psychotic BP and subtypes such as mood-incongruent psychotic BP have uncovered modest positive results for several candidate schizophrenia susceptibility genes, including dysbindin, DAOA/G30, Disrupted-in-Schizophrenia-1, and neuregulin 1. These tentative results are consistent with the hypothesis that the subphenotype of psychotic BP may represent a clinical manifestation of 'overlap' genes between schizophrenia and mood disorder syndromes.	topic_bd
78027	15	356222	7	NULL	NULL	0	NULL	neuregulin 1	GP		is a type of					schizophrenia susceptibility genes	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Psychotic features, defined as delusions or hallucinations, commonly occur in bipolar disorder (BP) and may be indicative of a more homogeneous form of the illness, with possible etiologic ties to schizophrenia. Several studies have shown that psychotic features aggregate in bipolar families, and increased interest in the molecular genetics of psychotic BP is emerging. Although preliminary, linkage studies of psychotic BP show replicated evidence for suggestive genome-wide linkage to chromosomes 8p and 13q, which have been implicated in prior linkage studies of schizophrenia and BP. Association studies of psychotic BP and subtypes such as mood-incongruent psychotic BP have uncovered modest positive results for several candidate schizophrenia susceptibility genes, including dysbindin, DAOA/G30, Disrupted-in-Schizophrenia-1, and neuregulin 1. These tentative results are consistent with the hypothesis that the subphenotype of psychotic BP may represent a clinical manifestation of 'overlap' genes between schizophrenia and mood disorder syndromes.	topic_bd
77782	1	356223	7	NULL	NULL	0	NULL	SIAT4A	GP		associated with					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	RESULTS: No genes specifically chosen to probe the action of lithium were associated with bipolar disorder. However, gene-based analysis of sialyltransferase 4A (SIAT4A), tachykinin receptor 1 (TACR1), and gamma-aminobutyric acid(A) beta2 receptor subunit (GABRB2) yielded evidence of association (empirical P value, <.005). Among 3 genes associated with schizophrenia or bipolar disorder in multiple previous studies, including dysbindin (DTNBP1), neuregulin (NRG1), and disrupted-in-schizophrenia 1 (DISC1), only DISC1 showed evidence of association in this cohort. In a secondary analysis of these 6 genes among parent-proband trios with a history of psychosis, evidence of the association with SIAT4A was strengthened.	topic_bd
77783	2	356223	7	NULL	NULL	0	NULL	TACR1	GP		associated with					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	RESULTS: No genes specifically chosen to probe the action of lithium were associated with bipolar disorder. However, gene-based analysis of sialyltransferase 4A (SIAT4A), tachykinin receptor 1 (TACR1), and gamma-aminobutyric acid(A) beta2 receptor subunit (GABRB2) yielded evidence of association (empirical P value, <.005). Among 3 genes associated with schizophrenia or bipolar disorder in multiple previous studies, including dysbindin (DTNBP1), neuregulin (NRG1), and disrupted-in-schizophrenia 1 (DISC1), only DISC1 showed evidence of association in this cohort. In a secondary analysis of these 6 genes among parent-proband trios with a history of psychosis, evidence of the association with SIAT4A was strengthened.	topic_bd
77784	3	356223	7	NULL	NULL	0	NULL	GABRB2	GP		associated with					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	RESULTS: No genes specifically chosen to probe the action of lithium were associated with bipolar disorder. However, gene-based analysis of sialyltransferase 4A (SIAT4A), tachykinin receptor 1 (TACR1), and gamma-aminobutyric acid(A) beta2 receptor subunit (GABRB2) yielded evidence of association (empirical P value, <.005). Among 3 genes associated with schizophrenia or bipolar disorder in multiple previous studies, including dysbindin (DTNBP1), neuregulin (NRG1), and disrupted-in-schizophrenia 1 (DISC1), only DISC1 showed evidence of association in this cohort. In a secondary analysis of these 6 genes among parent-proband trios with a history of psychosis, evidence of the association with SIAT4A was strengthened.	topic_bd
77785	4	356223	7	NULL	NULL	0	NULL	DISC1	GP		associated with					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	RESULTS: No genes specifically chosen to probe the action of lithium were associated with bipolar disorder. However, gene-based analysis of sialyltransferase 4A (SIAT4A), tachykinin receptor 1 (TACR1), and gamma-aminobutyric acid(A) beta2 receptor subunit (GABRB2) yielded evidence of association (empirical P value, <.005). Among 3 genes associated with schizophrenia or bipolar disorder in multiple previous studies, including dysbindin (DTNBP1), neuregulin (NRG1), and disrupted-in-schizophrenia 1 (DISC1), only DISC1 showed evidence of association in this cohort. In a secondary analysis of these 6 genes among parent-proband trios with a history of psychosis, evidence of the association with SIAT4A was strengthened.	topic_bd
77786	5	356223	7	NULL	NULL	0	NULL	DISC1	GP		associated with					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	RESULTS: No genes specifically chosen to probe the action of lithium were associated with bipolar disorder. However, gene-based analysis of sialyltransferase 4A (SIAT4A), tachykinin receptor 1 (TACR1), and gamma-aminobutyric acid(A) beta2 receptor subunit (GABRB2) yielded evidence of association (empirical P value, <.005). Among 3 genes associated with schizophrenia or bipolar disorder in multiple previous studies, including dysbindin (DTNBP1), neuregulin (NRG1), and disrupted-in-schizophrenia 1 (DISC1), only DISC1 showed evidence of association in this cohort. In a secondary analysis of these 6 genes among parent-proband trios with a history of psychosis, evidence of the association with SIAT4A was strengthened.	topic_bd
77787	6	356223	7	NULL	NULL	0	NULL	SIAT4A	GP		is					sialyltransferase 4A	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	RESULTS: No genes specifically chosen to probe the action of lithium were associated with bipolar disorder. However, gene-based analysis of sialyltransferase 4A (SIAT4A), tachykinin receptor 1 (TACR1), and gamma-aminobutyric acid(A) beta2 receptor subunit (GABRB2) yielded evidence of association (empirical P value, <.005). Among 3 genes associated with schizophrenia or bipolar disorder in multiple previous studies, including dysbindin (DTNBP1), neuregulin (NRG1), and disrupted-in-schizophrenia 1 (DISC1), only DISC1 showed evidence of association in this cohort. In a secondary analysis of these 6 genes among parent-proband trios with a history of psychosis, evidence of the association with SIAT4A was strengthened.	topic_bd
77788	7	356223	7	NULL	NULL	0	NULL	TACR1	GP		is					tachykinin receptor 1	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	RESULTS: No genes specifically chosen to probe the action of lithium were associated with bipolar disorder. However, gene-based analysis of sialyltransferase 4A (SIAT4A), tachykinin receptor 1 (TACR1), and gamma-aminobutyric acid(A) beta2 receptor subunit (GABRB2) yielded evidence of association (empirical P value, <.005). Among 3 genes associated with schizophrenia or bipolar disorder in multiple previous studies, including dysbindin (DTNBP1), neuregulin (NRG1), and disrupted-in-schizophrenia 1 (DISC1), only DISC1 showed evidence of association in this cohort. In a secondary analysis of these 6 genes among parent-proband trios with a history of psychosis, evidence of the association with SIAT4A was strengthened.	topic_bd
77789	8	356223	7	NULL	NULL	0	NULL	GABRB2	GP		is					gamma-aminobutyric acid(A) beta2 receptor subunit 	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	RESULTS: No genes specifically chosen to probe the action of lithium were associated with bipolar disorder. However, gene-based analysis of sialyltransferase 4A (SIAT4A), tachykinin receptor 1 (TACR1), and gamma-aminobutyric acid(A) beta2 receptor subunit (GABRB2) yielded evidence of association (empirical P value, <.005). Among 3 genes associated with schizophrenia or bipolar disorder in multiple previous studies, including dysbindin (DTNBP1), neuregulin (NRG1), and disrupted-in-schizophrenia 1 (DISC1), only DISC1 showed evidence of association in this cohort. In a secondary analysis of these 6 genes among parent-proband trios with a history of psychosis, evidence of the association with SIAT4A was strengthened.	topic_bd
77790	9	356223	7	NULL	NULL	0	NULL	DISC1	GP		is					disrupted-in-schizophrenia 1	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	RESULTS: No genes specifically chosen to probe the action of lithium were associated with bipolar disorder. However, gene-based analysis of sialyltransferase 4A (SIAT4A), tachykinin receptor 1 (TACR1), and gamma-aminobutyric acid(A) beta2 receptor subunit (GABRB2) yielded evidence of association (empirical P value, <.005). Among 3 genes associated with schizophrenia or bipolar disorder in multiple previous studies, including dysbindin (DTNBP1), neuregulin (NRG1), and disrupted-in-schizophrenia 1 (DISC1), only DISC1 showed evidence of association in this cohort. In a secondary analysis of these 6 genes among parent-proband trios with a history of psychosis, evidence of the association with SIAT4A was strengthened.	topic_bd
78415	1	356224	5	NULL	NULL	0	NULL	gray matter	OrganismPart	volume of	reduced in					pars opercularis	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	A significant gray matter volume reduction of both the pars opercularis and triangularis was found bilaterally in the subjects with ASD compared with the typical control subjects	topic_aut
78416	2	356224	5	NULL	NULL	0	NULL	gray matter	OrganismPart	volume of	reduced in					triangularis	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	A significant gray matter volume reduction of both the pars opercularis and triangularis was found bilaterally in the subjects with ASD compared with the typical control subjects	topic_aut
78417	3	356224	5	NULL	NULL	0	NULL	statement 1	Process		is present in					ASD subjects	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	A significant gray matter volume reduction of both the pars opercularis and triangularis was found bilaterally in the subjects with ASD compared with the typical control subjects	topic_aut
78418	4	356224	5	NULL	NULL	0	NULL	statement 2	Process		is present in					ASD subjects	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	A significant gray matter volume reduction of both the pars opercularis and triangularis was found bilaterally in the subjects with ASD compared with the typical control subjects	topic_aut
78419	1	356225	5	NULL	NULL	0	NULL	social communication	Process	severity of;;problems of	is increased in					ASD group	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	The reduced volume of right as well as total pars opercularis showed a significant association with the increased severity of social communication problems in the ASD group	topic_aut
78420	2	356225	5	NULL	NULL	0	NULL	pars opercularis	OrganismPart	reduced volume of;;right	is associated with		significantly			statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The reduced volume of right as well as total pars opercularis showed a significant association with the increased severity of social communication problems in the ASD group	topic_aut
78421	3	356225	5	NULL	NULL	0	NULL	pars opercularis	OrganismPart	reduced volume of;;total	is associated with		significantly			statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The reduced volume of right as well as total pars opercularis showed a significant association with the increased severity of social communication problems in the ASD group	topic_aut
78422	1	356226	5	NULL	NULL	0	NULL	imitation	Process		is a type of					MN related function	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Promising research has identified that interventions targeting MN related functions such as imitation can improve social functioning in ASDs	topic_aut
78423	2	356226	5	NULL	NULL	0	NULL	interventions	Process		target					MN related function	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Promising research has identified that interventions targeting MN related functions such as imitation can improve social functioning in ASDs	topic_aut
78424	3	356226	5	NULL	NULL	0	NULL	statement 2	Process		improves					social functioning	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Promising research has identified that interventions targeting MN related functions such as imitation can improve social functioning in ASDs	topic_aut
78425	4	356226	5	NULL	NULL	0	NULL	statement 3	Process		occurs in					ASDs	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Promising research has identified that interventions targeting MN related functions such as imitation can improve social functioning in ASDs	topic_aut
77791	1	356230	7	NULL	NULL	0	NULL	bipolar disorder	MedicalFinding		risky combination with					cardiometabolic diseases	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	'Bipolar disorder and cardiometabolic diseases- a risky combination' F. Laghrissi-Thode 9th International Conference on Bipolar Disorder	topic_bd
77792	1	356231	7	NULL	NULL	NULL	NULL	Obesity	MedicalFinding		involves					body fat	PhysicalPhenomenon	accumulation of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Obesity is a medical condition in which excess body fat has accumulated to the extent that it may have an adverse effect on health. It is defined by body mass index (BMI) and further evaluated in terms of fat distribution via the waist–hip ratio and total cardiovascular risk factors.	topic_bd
77793	2	356231	7	NULL	NULL	0	NULL	statement 1	Process		adverse effect on		may have			health	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity is a medical condition in which excess body fat has accumulated to the extent that it may have an adverse effect on health. It is defined by body mass index (BMI) and further evaluated in terms of fat distribution via the waist–hip ratio and total cardiovascular risk factors.	topic_bd
77794	3	356231	7	NULL	NULL	0	NULL	Obesity	MedicalFinding		is defined by					BMI	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity is a medical condition in which excess body fat has accumulated to the extent that it may have an adverse effect on health. It is defined by body mass index (BMI) and further evaluated in terms of fat distribution via the waist–hip ratio and total cardiovascular risk factors.	topic_bd
77795	4	356231	7	NULL	NULL	0	NULL	BMI	PhysicalPhenomenon		is					body mass index	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity is a medical condition in which excess body fat has accumulated to the extent that it may have an adverse effect on health. It is defined by body mass index (BMI) and further evaluated in terms of fat distribution via the waist–hip ratio and total cardiovascular risk factors.	topic_bd
77796	1	356234	7	NULL	NULL	NULL	NULL	immunoglobulin	GP		is a type of					large Y-shaped protein	GP				NULL		NULL	NULL	NULL	NULL	NULL	NULL	An antibody, also known as an immunoglobulin, is a large Y-shaped protein used by the immune system to identify and neutralize foreign objects such as bacteria and viruses.	topic_bd
77797	2	356234	7	NULL	NULL	0	NULL	Antibody	GP		also known as					immunoglobulin	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	An antibody, also known as an immunoglobulin, is a large Y-shaped protein used by the immune system to identify and neutralize foreign objects such as bacteria and viruses.	topic_bd
77798	3	356234	7	NULL	NULL	0	NULL	immunoglobulin	GP		used by					immune system	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	An antibody, also known as an immunoglobulin, is a large Y-shaped protein used by the immune system to identify and neutralize foreign objects such as bacteria and viruses.	topic_bd
77799	4	356234	7	NULL	NULL	0	NULL	immunoglobulin	GP		identify					bacteria	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	An antibody, also known as an immunoglobulin, is a large Y-shaped protein used by the immune system to identify and neutralize foreign objects such as bacteria and viruses.	topic_bd
77800	5	356234	7	NULL	NULL	0	NULL	immunoglobulin	GP		identify					virus	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	An antibody, also known as an immunoglobulin, is a large Y-shaped protein used by the immune system to identify and neutralize foreign objects such as bacteria and viruses.	topic_bd
77801	6	356234	7	NULL	NULL	NULL	NULL	immunoglobulin	GP		neutralize					bacteria	Organism				NULL		NULL	NULL	NULL	NULL	NULL	NULL	An antibody, also known as an immunoglobulin, is a large Y-shaped protein used by the immune system to identify and neutralize foreign objects such as bacteria and viruses.	topic_bd
77802	7	356234	7	NULL	NULL	0	NULL	statement 4	Process		occur with					statement 6	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	An antibody, also known as an immunoglobulin, is a large Y-shaped protein used by the immune system to identify and neutralize foreign objects such as bacteria and viruses.	topic_bd
77803	8	356234	7	NULL	NULL	0	NULL	immunoglobulin	GP		neutralize					virus	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	An antibody, also known as an immunoglobulin, is a large Y-shaped protein used by the immune system to identify and neutralize foreign objects such as bacteria and viruses.	topic_bd
77804	9	356234	7	NULL	NULL	0	NULL	statement 5	Process		occur with					statement 8	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	An antibody, also known as an immunoglobulin, is a large Y-shaped protein used by the immune system to identify and neutralize foreign objects such as bacteria and viruses.	topic_bd
77805	10	356234	7	NULL	NULL	0	NULL	bacteria	Organism		is a type of					foreign object	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	An antibody, also known as an immunoglobulin, is a large Y-shaped protein used by the immune system to identify and neutralize foreign objects such as bacteria and viruses.	topic_bd
77806	11	356234	7	NULL	NULL	0	NULL	virus	Organism		is a type of					foreign object	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	An antibody, also known as an immunoglobulin, is a large Y-shaped protein used by the immune system to identify and neutralize foreign objects such as bacteria and viruses.	topic_bd
77807	1	356235	7	NULL	NULL	0	NULL	NMDAR	GP		is a type of					glutamate receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The NMDA receptor (NMDAR), a glutamate receptor, is the predominant molecular device for controlling synaptic plasticity and memory function.	topic_bd
77808	2	356235	7	NULL	NULL	0	NULL	NMDAR	GP		predominant					synaptic plasticity 	Process	molecular device for controlling			NULL		0	NULL	NULL	NULL	NULL	NULL	The NMDA receptor (NMDAR), a glutamate receptor, is the predominant molecular device for controlling synaptic plasticity and memory function.	topic_bd
77809	3	356235	7	NULL	NULL	0	NULL	NMDAR	GP		predominant					memory function	Process	molecular device for controlling			NULL		0	NULL	NULL	NULL	NULL	NULL	The NMDA receptor (NMDAR), a glutamate receptor, is the predominant molecular device for controlling synaptic plasticity and memory function.	topic_bd
77810	4	356235	7	NULL	NULL	0	NULL	NMDAR	GP		is					NMDA receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The NMDA receptor (NMDAR), a glutamate receptor, is the predominant molecular device for controlling synaptic plasticity and memory function.	topic_bd
77811	1	356236	7	NULL	NULL	0	NULL	Glutamic acid	AminoAcid		is a type of					 20 proteinogenic amino acids	AminoAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamic acid (abbreviated as Glu or E) is one of the 20 proteinogenic amino acids, and its codons are GAA and GAG. It is a non-essential amino acid. The carboxylate anions and salts of glutamic acid are known as glutamates. In neuroscience, glutamate is an important neurotransmitter that plays a key role in long-term potentiation and is important for learning and memory.	topic_bd
77812	2	356236	7	NULL	NULL	0	NULL	GAA	GP		codon for					Glutamic acid	AminoAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamic acid (abbreviated as Glu or E) is one of the 20 proteinogenic amino acids, and its codons are GAA and GAG. It is a non-essential amino acid. The carboxylate anions and salts of glutamic acid are known as glutamates. In neuroscience, glutamate is an important neurotransmitter that plays a key role in long-term potentiation and is important for learning and memory.	topic_bd
77813	3	356236	7	NULL	NULL	0	NULL	GAG	GP		codon for					Glutamic acid	AminoAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamic acid (abbreviated as Glu or E) is one of the 20 proteinogenic amino acids, and its codons are GAA and GAG. It is a non-essential amino acid. The carboxylate anions and salts of glutamic acid are known as glutamates. In neuroscience, glutamate is an important neurotransmitter that plays a key role in long-term potentiation and is important for learning and memory.	topic_bd
77814	4	356236	7	NULL	NULL	0	NULL	Glutamic acid	AminoAcid		abbreviated as					Glu	AminoAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamic acid (abbreviated as Glu or E) is one of the 20 proteinogenic amino acids, and its codons are GAA and GAG. It is a non-essential amino acid. The carboxylate anions and salts of glutamic acid are known as glutamates. In neuroscience, glutamate is an important neurotransmitter that plays a key role in long-term potentiation and is important for learning and memory.	topic_bd
77815	5	356236	7	NULL	NULL	0	NULL	Glutamic acid	AminoAcid		abbreviated as					E	AminoAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamic acid (abbreviated as Glu or E) is one of the 20 proteinogenic amino acids, and its codons are GAA and GAG. It is a non-essential amino acid. The carboxylate anions and salts of glutamic acid are known as glutamates. In neuroscience, glutamate is an important neurotransmitter that plays a key role in long-term potentiation and is important for learning and memory.	topic_bd
77816	6	356236	7	NULL	NULL	0	NULL	Glu	AminoAcid		is a type of					non-essential amino acid	AminoAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamic acid (abbreviated as Glu or E) is one of the 20 proteinogenic amino acids, and its codons are GAA and GAG. It is a non-essential amino acid. The carboxylate anions and salts of glutamic acid are known as glutamates. In neuroscience, glutamate is an important neurotransmitter that plays a key role in long-term potentiation and is important for learning and memory.	topic_bd
77817	7	356236	7	NULL	NULL	NULL	NULL	Glutamic acid	AminoAcid	carboxylate anions of	known as					glutamates	Chemical				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glutamic acid (abbreviated as Glu or E) is one of the 20 proteinogenic amino acids, and its codons are GAA and GAG. It is a non-essential amino acid. The carboxylate anions and salts of glutamic acid are known as glutamates. In neuroscience, glutamate is an important neurotransmitter that plays a key role in long-term potentiation and is important for learning and memory.	topic_bd
77818	8	356236	7	NULL	NULL	NULL	NULL	Glutamic acid	AminoAcid	salts of	known as					glutamates	Chemical				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glutamic acid (abbreviated as Glu or E) is one of the 20 proteinogenic amino acids, and its codons are GAA and GAG. It is a non-essential amino acid. The carboxylate anions and salts of glutamic acid are known as glutamates. In neuroscience, glutamate is an important neurotransmitter that plays a key role in long-term potentiation and is important for learning and memory.	topic_bd
77819	9	356236	7	NULL	NULL	0	NULL	glutamate	Chemical		is an important					neurotransmitter	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamic acid (abbreviated as Glu or E) is one of the 20 proteinogenic amino acids, and its codons are GAA and GAG. It is a non-essential amino acid. The carboxylate anions and salts of glutamic acid are known as glutamates. In neuroscience, glutamate is an important neurotransmitter that plays a key role in long-term potentiation and is important for learning and memory.	topic_bd
77820	10	356236	7	NULL	NULL	0	NULL	glutamate	Chemical		play					long-term potentiation	Process	key role in			NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamic acid (abbreviated as Glu or E) is one of the 20 proteinogenic amino acids, and its codons are GAA and GAG. It is a non-essential amino acid. The carboxylate anions and salts of glutamic acid are known as glutamates. In neuroscience, glutamate is an important neurotransmitter that plays a key role in long-term potentiation and is important for learning and memory.	topic_bd
77821	11	356236	7	NULL	NULL	0	NULL	glutamate	Chemical		is important for					learning	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamic acid (abbreviated as Glu or E) is one of the 20 proteinogenic amino acids, and its codons are GAA and GAG. It is a non-essential amino acid. The carboxylate anions and salts of glutamic acid are known as glutamates. In neuroscience, glutamate is an important neurotransmitter that plays a key role in long-term potentiation and is important for learning and memory.	topic_bd
77822	12	356236	7	NULL	NULL	0	NULL	glutamate	Chemical		is important for					memory	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamic acid (abbreviated as Glu or E) is one of the 20 proteinogenic amino acids, and its codons are GAA and GAG. It is a non-essential amino acid. The carboxylate anions and salts of glutamic acid are known as glutamates. In neuroscience, glutamate is an important neurotransmitter that plays a key role in long-term potentiation and is important for learning and memory.	topic_bd
77823	1	356237	7	NULL	NULL	0	NULL	Mitochondrial dysfunction	Process		occur in					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	"Mitochondrial dysfunction and oxidative stress in bipolar disorder" LT Young 9th International Conference on Bipolar Disorder	topic_bd
77824	2	356237	7	NULL	NULL	0	NULL	oxidative stress	Process		occur in					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	"Mitochondrial dysfunction and oxidative stress in bipolar disorder" LT Young 9th International Conference on Bipolar Disorder	topic_bd
77825	1	356238	7	NULL	NULL	0	NULL	reactive oxygen species	Chemical	production of	imbalance with					Reactive oxygen species 	Chemical	manifestation of			NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidative stress represents an imbalance between the production and manifestation of reactive oxygen species and a biological system's ability to readily detoxify the reactive intermediates or to repair the resulting damage.	topic_bd
77826	2	356238	7	NULL	NULL	0	NULL	oxidative stress	Process		represents					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidative stress represents an imbalance between the production and manifestation of reactive oxygen species and a biological system's ability to readily detoxify the reactive intermediates or to repair the resulting damage.	topic_bd
77827	3	356238	7	NULL	NULL	0	NULL	biological system	Process		detoxify		readily			reactive intermediates	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidative stress represents an imbalance between the production and manifestation of reactive oxygen species and a biological system's ability to readily detoxify the reactive intermediates or to repair the resulting damage.	topic_bd
77828	4	356238	7	NULL	NULL	NULL	NULL	oxidative stress	Process		represents					statement 3	Process	ability of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Oxidative stress represents an imbalance between the production and manifestation of reactive oxygen species and a biological system's ability to readily detoxify the reactive intermediates or to repair the resulting damage.	topic_bd
77829	5	356238	7	NULL	NULL	0	NULL	biological system	Process		repair					 damage	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidative stress represents an imbalance between the production and manifestation of reactive oxygen species and a biological system's ability to readily detoxify the reactive intermediates or to repair the resulting damage.	topic_bd
77830	6	356238	7	NULL	NULL	0	NULL	oxidative stress	Process		represents					statement 5	Process	ability of			NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidative stress represents an imbalance between the production and manifestation of reactive oxygen species and a biological system's ability to readily detoxify the reactive intermediates or to repair the resulting damage.	topic_bd
77831	7	356238	7	NULL	NULL	0	NULL	statement 4	Process		is an alternative to					statement 6	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidative stress represents an imbalance between the production and manifestation of reactive oxygen species and a biological system's ability to readily detoxify the reactive intermediates or to repair the resulting damage.	topic_bd
77832	1	356239	7	NULL	NULL	0	NULL	Radicals	Chemical		referred to as					free radicals	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Radicals (often referred to as free radicals) are atoms, molecules, or ions with unpaired electrons on an open shell configuration. Free radicals may have positive, negative, or zero charge. With some exceptions, the unpaired electrons cause radicals to be highly chemically reactive. Radicals, if allowed to run free in the body, are believed to be involved in degenerative diseases and cancers.	topic_bd
77833	2	356239	7	NULL	NULL	0	NULL	Radicals	Chemical		is a type of					atoms	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Radicals (often referred to as free radicals) are atoms, molecules, or ions with unpaired electrons on an open shell configuration. Free radicals may have positive, negative, or zero charge. With some exceptions, the unpaired electrons cause radicals to be highly chemically reactive. Radicals, if allowed to run free in the body, are believed to be involved in degenerative diseases and cancers.	topic_bd
77834	3	356239	7	NULL	NULL	0	NULL	Radicals	Chemical		is a type of					molecule	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Radicals (often referred to as free radicals) are atoms, molecules, or ions with unpaired electrons on an open shell configuration. Free radicals may have positive, negative, or zero charge. With some exceptions, the unpaired electrons cause radicals to be highly chemically reactive. Radicals, if allowed to run free in the body, are believed to be involved in degenerative diseases and cancers.	topic_bd
77835	5	356239	7	NULL	NULL	NULL	NULL	Radicals	Chemical		is a type of					statement 4	Chemical				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Radicals (often referred to as free radicals) are atoms, molecules, or ions with unpaired electrons on an open shell configuration. Free radicals may have positive, negative, or zero charge. With some exceptions, the unpaired electrons cause radicals to be highly chemically reactive. Radicals, if allowed to run free in the body, are believed to be involved in degenerative diseases and cancers.	topic_bd
77836	4	356239	7	NULL	NULL	NULL	NULL	ions	Chemical		contain					unpaired electron	Chemical	an open shell configuration			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Radicals (often referred to as free radicals) are atoms, molecules, or ions with unpaired electrons on an open shell configuration. Free radicals may have positive, negative, or zero charge. With some exceptions, the unpaired electrons cause radicals to be highly chemically reactive. Radicals, if allowed to run free in the body, are believed to be involved in degenerative diseases and cancers.	topic_bd
77837	6	356239	7	NULL	NULL	0	NULL	free radicals	Chemical		have		may			positive charge	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Radicals (often referred to as free radicals) are atoms, molecules, or ions with unpaired electrons on an open shell configuration. Free radicals may have positive, negative, or zero charge. With some exceptions, the unpaired electrons cause radicals to be highly chemically reactive. Radicals, if allowed to run free in the body, are believed to be involved in degenerative diseases and cancers.	topic_bd
77838	7	356239	7	NULL	NULL	0	NULL	free radicals	Chemical		have		may			negative charge	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Radicals (often referred to as free radicals) are atoms, molecules, or ions with unpaired electrons on an open shell configuration. Free radicals may have positive, negative, or zero charge. With some exceptions, the unpaired electrons cause radicals to be highly chemically reactive. Radicals, if allowed to run free in the body, are believed to be involved in degenerative diseases and cancers.	topic_bd
77839	8	356239	7	NULL	NULL	0	NULL	free radicals	Chemical		have		may			zero charge	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Radicals (often referred to as free radicals) are atoms, molecules, or ions with unpaired electrons on an open shell configuration. Free radicals may have positive, negative, or zero charge. With some exceptions, the unpaired electrons cause radicals to be highly chemically reactive. Radicals, if allowed to run free in the body, are believed to be involved in degenerative diseases and cancers.	topic_bd
77840	9	356239	7	NULL	NULL	0	NULL	radicals	Chemical		chemically		highly			reactive	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Radicals (often referred to as free radicals) are atoms, molecules, or ions with unpaired electrons on an open shell configuration. Free radicals may have positive, negative, or zero charge. With some exceptions, the unpaired electrons cause radicals to be highly chemically reactive. Radicals, if allowed to run free in the body, are believed to be involved in degenerative diseases and cancers.	topic_bd
77841	10	356239	7	NULL	NULL	0	NULL	unpaired electrons	Chemical		cause					statement 9	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Radicals (often referred to as free radicals) are atoms, molecules, or ions with unpaired electrons on an open shell configuration. Free radicals may have positive, negative, or zero charge. With some exceptions, the unpaired electrons cause radicals to be highly chemically reactive. Radicals, if allowed to run free in the body, are believed to be involved in degenerative diseases and cancers.	topic_bd
77842	11	356239	7	NULL	NULL	0	NULL	radicals	Chemical		involved in					 degenerative diseases 	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Radicals (often referred to as free radicals) are atoms, molecules, or ions with unpaired electrons on an open shell configuration. Free radicals may have positive, negative, or zero charge. With some exceptions, the unpaired electrons cause radicals to be highly chemically reactive. Radicals, if allowed to run free in the body, are believed to be involved in degenerative diseases and cancers.	topic_bd
77843	12	356239	7	NULL	NULL	0	NULL	radicals	Chemical		involved in					cancers	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Radicals (often referred to as free radicals) are atoms, molecules, or ions with unpaired electrons on an open shell configuration. Free radicals may have positive, negative, or zero charge. With some exceptions, the unpaired electrons cause radicals to be highly chemically reactive. Radicals, if allowed to run free in the body, are believed to be involved in degenerative diseases and cancers.	topic_bd
77844	13	356239	7	NULL	NULL	0	NULL	statement 6	Process		is an alternative to					statement 7	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Radicals (often referred to as free radicals) are atoms, molecules, or ions with unpaired electrons on an open shell configuration. Free radicals may have positive, negative, or zero charge. With some exceptions, the unpaired electrons cause radicals to be highly chemically reactive. Radicals, if allowed to run free in the body, are believed to be involved in degenerative diseases and cancers.	topic_bd
77845	14	356239	7	NULL	NULL	0	NULL	statement 6	Process		is an alternative to					statement 8	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Radicals (often referred to as free radicals) are atoms, molecules, or ions with unpaired electrons on an open shell configuration. Free radicals may have positive, negative, or zero charge. With some exceptions, the unpaired electrons cause radicals to be highly chemically reactive. Radicals, if allowed to run free in the body, are believed to be involved in degenerative diseases and cancers.	topic_bd
77846	1	356241	7	NULL	NULL	0	NULL	glutamate	Chemical		is involved in					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The neurotransmitter glutamate is thought to be involved in bipolar disorder.	topic_bd
77847	2	356241	7	NULL	NULL	0	NULL	glutamate	Chemical		is a type of					neurotransmitter	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The neurotransmitter glutamate is thought to be involved in bipolar disorder.	topic_bd
77848	1	356242	7	NULL	NULL	0	NULL	Body mass index	PhysicalPhenomenon		associated with		positively			CRC	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	Body mass index in early adulthood is positively associated with risk of CRC for MMR gene mutation carriers and non-carriers.British Journal of Cancer advance online publication	topic_ccc
77849	2	356242	7	NULL	NULL	0	NULL	statement 1	Process		occur in					MMR gene mutation carriers	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Body mass index in early adulthood is positively associated with risk of CRC for MMR gene mutation carriers and non-carriers.British Journal of Cancer advance online publication	topic_ccc
77850	3	356242	7	NULL	NULL	0	NULL	statement 1	Process		occur in					MMR gene mutation non-carriers	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Body mass index in early adulthood is positively associated with risk of CRC for MMR gene mutation carriers and non-carriers.British Journal of Cancer advance online publication	topic_ccc
77851	4	356242	7	NULL	NULL	0	NULL	statement 1	Process		occur in					early adulthood	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	NULL	NULL	Body mass index in early adulthood is positively associated with risk of CRC for MMR gene mutation carriers and non-carriers.British Journal of Cancer advance online publication	topic_ccc
78001	1	356245	7	NULL	NULL	NULL	NULL	cytokines	Chemical		is a type of					cell-signaling protein molecules	GP	small			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytokines (Greek cyto-, cell; and -kinos, movement) are small cell-signaling protein molecules that are secreted by the glial cells of the nervous system and by numerous cells of the immune system and are a category of signaling molecules used extensively in intercellular communication. Cytokines can be classified as proteins, peptides, or glycoproteins; the term "cytokine" encompasses a large and diverse family of regulators produced throughout the body by cells of diverse embryological origin.[1]	topic_bd
78002	2	356245	7	NULL	NULL	0	NULL	statement 1	Process		secreted by					nervous system	OrganismPart	glial cells of			NULL		0	NULL	NULL	NULL	NULL	NULL	Cytokines (Greek cyto-, cell; and -kinos, movement) are small cell-signaling protein molecules that are secreted by the glial cells of the nervous system and by numerous cells of the immune system and are a category of signaling molecules used extensively in intercellular communication. Cytokines can be classified as proteins, peptides, or glycoproteins; the term "cytokine" encompasses a large and diverse family of regulators produced throughout the body by cells of diverse embryological origin.[1]	topic_bd
78003	3	356245	7	NULL	NULL	NULL	NULL	statement 1	Process		secreted by					immune system	OrganismPart	cells of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytokines (Greek cyto-, cell; and -kinos, movement) are small cell-signaling protein molecules that are secreted by the glial cells of the nervous system and by numerous cells of the immune system and are a category of signaling molecules used extensively in intercellular communication. Cytokines can be classified as proteins, peptides, or glycoproteins; the term "cytokine" encompasses a large and diverse family of regulators produced throughout the body by cells of diverse embryological origin.[1]	topic_bd
78004	4	356245	7	NULL	NULL	0	NULL	cytokines	Chemical		used in		extensively			intercellular communication	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Cytokines (Greek cyto-, cell; and -kinos, movement) are small cell-signaling protein molecules that are secreted by the glial cells of the nervous system and by numerous cells of the immune system and are a category of signaling molecules used extensively in intercellular communication. Cytokines can be classified as proteins, peptides, or glycoproteins; the term "cytokine" encompasses a large and diverse family of regulators produced throughout the body by cells of diverse embryological origin.[1]	topic_bd
78005	5	356245	7	NULL	NULL	0	NULL	cytokines	Chemical		classified  as					proteins	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Cytokines (Greek cyto-, cell; and -kinos, movement) are small cell-signaling protein molecules that are secreted by the glial cells of the nervous system and by numerous cells of the immune system and are a category of signaling molecules used extensively in intercellular communication. Cytokines can be classified as proteins, peptides, or glycoproteins; the term "cytokine" encompasses a large and diverse family of regulators produced throughout the body by cells of diverse embryological origin.[1]	topic_bd
78006	6	356245	7	NULL	NULL	0	NULL	cytokines	Chemical		classified  as					peptides	AminoAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	Cytokines (Greek cyto-, cell; and -kinos, movement) are small cell-signaling protein molecules that are secreted by the glial cells of the nervous system and by numerous cells of the immune system and are a category of signaling molecules used extensively in intercellular communication. Cytokines can be classified as proteins, peptides, or glycoproteins; the term "cytokine" encompasses a large and diverse family of regulators produced throughout the body by cells of diverse embryological origin.[1]	topic_bd
78007	7	356245	7	NULL	NULL	0	NULL	cytokines	Chemical		classified  as					glycoproteins	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Cytokines (Greek cyto-, cell; and -kinos, movement) are small cell-signaling protein molecules that are secreted by the glial cells of the nervous system and by numerous cells of the immune system and are a category of signaling molecules used extensively in intercellular communication. Cytokines can be classified as proteins, peptides, or glycoproteins; the term "cytokine" encompasses a large and diverse family of regulators produced throughout the body by cells of diverse embryological origin.[1]	topic_bd
78008	8	356245	7	NULL	NULL	NULL	NULL	cytokines	Chemical		encompasses					regulators	Chemical	large and diverse family of 			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytokines (Greek cyto-, cell; and -kinos, movement) are small cell-signaling protein molecules that are secreted by the glial cells of the nervous system and by numerous cells of the immune system and are a category of signaling molecules used extensively in intercellular communication. Cytokines can be classified as proteins, peptides, or glycoproteins; the term "cytokine" encompasses a large and diverse family of regulators produced throughout the body by cells of diverse embryological origin.[1]	topic_bd
78009	9	356245	7	NULL	NULL	0	NULL	cytokines	Chemical		produced					embryological origin	OrganismPart	throughout the body cells of diverse			NULL		0	NULL	NULL	NULL	NULL	NULL	Cytokines (Greek cyto-, cell; and -kinos, movement) are small cell-signaling protein molecules that are secreted by the glial cells of the nervous system and by numerous cells of the immune system and are a category of signaling molecules used extensively in intercellular communication. Cytokines can be classified as proteins, peptides, or glycoproteins; the term "cytokine" encompasses a large and diverse family of regulators produced throughout the body by cells of diverse embryological origin.[1]	topic_bd
78010	1	356246	7	NULL	NULL	0	NULL	Somatic treatment	MedicalProcedure		treatment of					physical means	MedicalProcedure	mental illness by			NULL		0	NULL	NULL	NULL	NULL	NULL	Somatic treatment is the treatment of mental illness by physical means (such as medication, electroconvulsive therapy, or psychosurgery) rather than psychotherapy.	topic_bd
78011	2	356246	7	NULL	NULL	0	NULL	physical means	MedicalProcedure		include					medication	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Somatic treatment is the treatment of mental illness by physical means (such as medication, electroconvulsive therapy, or psychosurgery) rather than psychotherapy.	topic_bd
78012	3	356246	7	NULL	NULL	0	NULL	physical means	MedicalProcedure		include					electroconvulsive therapy	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Somatic treatment is the treatment of mental illness by physical means (such as medication, electroconvulsive therapy, or psychosurgery) rather than psychotherapy.	topic_bd
78013	4	356246	7	NULL	NULL	0	NULL	physical means	MedicalProcedure		include					 psychosurgery	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Somatic treatment is the treatment of mental illness by physical means (such as medication, electroconvulsive therapy, or psychosurgery) rather than psychotherapy.	topic_bd
78014	5	356246	7	NULL	NULL	0	NULL	physical means	MedicalProcedure		does not mean					psychotherapy	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Somatic treatment is the treatment of mental illness by physical means (such as medication, electroconvulsive therapy, or psychosurgery) rather than psychotherapy.	topic_bd
77852	1	356247	7	NULL	NULL	0	NULL	cerebral cortex	OrganismPart	 temporal lobe of	located beneath					Sylvian fissure	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	The temporal lobe is a region of the cerebral cortex that is located beneath the Sylvian fissure on both cerebral hemispheres of the mammalian brain.	topic_bd
77853	2	356247	7	NULL	NULL	0	NULL	statement 1	Process		present on					mammalian brain	OrganismPart	cerebral hemispheres of			NULL		0	NULL	NULL	NULL	NULL	NULL	The temporal lobe is a region of the cerebral cortex that is located beneath the Sylvian fissure on both cerebral hemispheres of the mammalian brain.	topic_bd
77854	1	356248	7	NULL	NULL	NULL	NULL	basal ganglia	OrganismPart		group of					nuclei	CellComponent				NULL		NULL	NULL	NULL	NULL	NULL	NULL	The basal ganglia (or basal nuclei) are a group of nuclei of varied origin (mostly telencephalic embryonal origin, with some diencephalic and mesencephalic elements) in the brains of vertebrates that act as a cohesive functional unit.	topic_bd
77855	2	356248	7	NULL	NULL	0	NULL	statement 1	Process		belongs to					telencephalic embryonal origin	CellComponent				NULL		0	NULL	NULL	NULL	NULL	NULL	The basal ganglia (or basal nuclei) are a group of nuclei of varied origin (mostly telencephalic embryonal origin, with some diencephalic and mesencephalic elements) in the brains of vertebrates that act as a cohesive functional unit.	topic_bd
77856	3	356248	7	NULL	NULL	0	NULL	statement 1	Process		belongs to					diencephalic element	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	The basal ganglia (or basal nuclei) are a group of nuclei of varied origin (mostly telencephalic embryonal origin, with some diencephalic and mesencephalic elements) in the brains of vertebrates that act as a cohesive functional unit.	topic_bd
77857	4	356248	7	NULL	NULL	0	NULL	statement 1	Process		belongs to					mesencephalic elements	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	The basal ganglia (or basal nuclei) are a group of nuclei of varied origin (mostly telencephalic embryonal origin, with some diencephalic and mesencephalic elements) in the brains of vertebrates that act as a cohesive functional unit.	topic_bd
77858	5	356248	7	NULL	NULL	0	NULL	basal ganglia	CellComponent		present in					vertebrates	Organism	brains of			NULL		0	NULL	NULL	NULL	NULL	NULL	The basal ganglia (or basal nuclei) are a group of nuclei of varied origin (mostly telencephalic embryonal origin, with some diencephalic and mesencephalic elements) in the brains of vertebrates that act as a cohesive functional unit.	topic_bd
77859	6	356248	7	NULL	NULL	0	NULL	basal ganglia	OrganismPart		act as a					cohesive functional unit	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	The basal ganglia (or basal nuclei) are a group of nuclei of varied origin (mostly telencephalic embryonal origin, with some diencephalic and mesencephalic elements) in the brains of vertebrates that act as a cohesive functional unit.	topic_bd
77860	1	356249	7	NULL	NULL	0	NULL	Thyroid disorders	MedicalFinding		include					hyperthyroidism 	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Thyroid disorders include hyperthyroidism (abnormally increased activity), hypothyroidism (abnormally decreased activity) and thyroid nodules, which are generally benign thyroid neoplasms, but may be thyroid cancers.	topic_bd
77861	2	356249	7	NULL	NULL	0	NULL	Thyroid disorders	MedicalFinding		include					hypothyroidism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Thyroid disorders include hyperthyroidism (abnormally increased activity), hypothyroidism (abnormally decreased activity) and thyroid nodules, which are generally benign thyroid neoplasms, but may be thyroid cancers.	topic_bd
77862	3	356249	7	NULL	NULL	0	NULL	Thyroid disorders	MedicalFinding		include					thyroid nodules	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Thyroid disorders include hyperthyroidism (abnormally increased activity), hypothyroidism (abnormally decreased activity) and thyroid nodules, which are generally benign thyroid neoplasms, but may be thyroid cancers.	topic_bd
77863	4	356249	7	NULL	NULL	0	NULL	thyroid nodules	OrganismPart		benign		generally			thyroid neoplasms	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Thyroid disorders include hyperthyroidism (abnormally increased activity), hypothyroidism (abnormally decreased activity) and thyroid nodules, which are generally benign thyroid neoplasms, but may be thyroid cancers.	topic_bd
77864	5	356249	7	NULL	NULL	0	NULL	thyroid neoplasms	OrganismPart		may be					thyroid cancers	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Thyroid disorders include hyperthyroidism (abnormally increased activity), hypothyroidism (abnormally decreased activity) and thyroid nodules, which are generally benign thyroid neoplasms, but may be thyroid cancers.	topic_bd
77865	6	356249	7	NULL	NULL	0	NULL	Hyperthyroidism	MedicalFinding		shows					abnormal increased activity	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Thyroid disorders include hyperthyroidism (abnormally increased activity), hypothyroidism (abnormally decreased activity) and thyroid nodules, which are generally benign thyroid neoplasms, but may be thyroid cancers.	topic_bd
77866	7	356249	7	NULL	NULL	0	NULL	Hypothyroidism 	MedicalFinding		shows					abnormal decreased activity	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Thyroid disorders include hyperthyroidism (abnormally increased activity), hypothyroidism (abnormally decreased activity) and thyroid nodules, which are generally benign thyroid neoplasms, but may be thyroid cancers.	topic_bd
77867	1	356250	7	NULL	NULL	0	NULL	thyroid gland	OrganismPart		is found in					neck	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	The thyroid gland is found in the neck, below (inferior to) the thyroid cartilage (which forms the laryngeal prominence, or 'Adam's Apple').	topic_bd
77868	2	356250	7	NULL	NULL	0	NULL	thyroid gland	OrganismPart		is found below					thyroid cartilage	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	The thyroid gland is found in the neck, below (inferior to) the thyroid cartilage (which forms the laryngeal prominence, or 'Adam's Apple').	topic_bd
77869	3	356250	7	NULL	NULL	0	NULL	thryoid cartilage	OrganismPart		forms					laryngeal prominence	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	The thyroid gland is found in the neck, below (inferior to) the thyroid cartilage (which forms the laryngeal prominence, or 'Adam's Apple').	topic_bd
77870	4	356250	7	NULL	NULL	0	NULL	laryngeal prominence	OrganismPart		is known as					Adam's apple	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	The thyroid gland is found in the neck, below (inferior to) the thyroid cartilage (which forms the laryngeal prominence, or 'Adam's Apple').	topic_bd
77871	1	356251	7	NULL	NULL	0	NULL	hypothalamus	OrganismPart		is a portion of					brain	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	The Hypothalamus  is a portion of the brain that contains a number of small nuclei with a variety of functions.	topic_bd
77872	2	356251	7	NULL	NULL	0	NULL	hypothalamus	OrganismPart		contains					small nuclei	CellComponent				NULL		0	NULL	NULL	NULL	NULL	NULL	The Hypothalamus  is a portion of the brain that contains a number of small nuclei with a variety of functions.	topic_bd
77873	1	356252	7	NULL	NULL	0	NULL	abnormal gene expression	Process		is defined as					gene	GP	transcription of below normal levels of			NULL		0	NULL	NULL	NULL	NULL	NULL	Abnormal gene expression is the transcription of a gene above or below normal levels.	topic_bd
77874	2	356252	7	NULL	NULL	NULL	NULL	abnormal gene expression	Process		is defined as					gene	GP	transcription of above normal levels of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Abnormal gene expression is the transcription of a gene above or below normal levels.	topic_bd
77875	1	356253	7	NULL	NULL	0	NULL	Bipolar disorder	MedicalFinding		referred to as					bipolar affective disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar disorder or manic–depressive disorder, also referred to as bipolar affective disorder or manic depression, is a psychiatric diagnosis that describes a category of mood disorders defined by the presence of one or more episodes of abnormally elevated energy levels, cognition, and mood with or without one or more depressive episodes.	topic_bd
77876	2	356253	7	NULL	NULL	0	NULL	manic depressive disorder	MedicalFinding		referred to as					manic depression 	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar disorder or manic–depressive disorder, also referred to as bipolar affective disorder or manic depression, is a psychiatric diagnosis that describes a category of mood disorders defined by the presence of one or more episodes of abnormally elevated energy levels, cognition, and mood with or without one or more depressive episodes.	topic_bd
77877	3	356253	7	NULL	NULL	0	NULL	bipolar disorder	MedicalFinding		is a type of					psychiatric diagnosis	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar disorder or manic–depressive disorder, also referred to as bipolar affective disorder or manic depression, is a psychiatric diagnosis that describes a category of mood disorders defined by the presence of one or more episodes of abnormally elevated energy levels, cognition, and mood with or without one or more depressive episodes.	topic_bd
77878	4	356253	7	NULL	NULL	0	NULL	manic depressive disorder	MedicalFinding		is a type of					psychiatric diagnosis	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar disorder or manic–depressive disorder, also referred to as bipolar affective disorder or manic depression, is a psychiatric diagnosis that describes a category of mood disorders defined by the presence of one or more episodes of abnormally elevated energy levels, cognition, and mood with or without one or more depressive episodes.	topic_bd
77879	5	356253	7	NULL	NULL	0	NULL	bipolar disorder	MedicalFinding		describes					mood disorders	MedicalFinding	category of			NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar disorder or manic–depressive disorder, also referred to as bipolar affective disorder or manic depression, is a psychiatric diagnosis that describes a category of mood disorders defined by the presence of one or more episodes of abnormally elevated energy levels, cognition, and mood with or without one or more depressive episodes.	topic_bd
77880	6	356253	7	NULL	NULL	0	NULL	mood disorders	MedicalFinding		defined by					energy levels	MentalProcess	episodes of abnormally elevated			NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar disorder or manic–depressive disorder, also referred to as bipolar affective disorder or manic depression, is a psychiatric diagnosis that describes a category of mood disorders defined by the presence of one or more episodes of abnormally elevated energy levels, cognition, and mood with or without one or more depressive episodes.	topic_bd
77881	7	356253	7	NULL	NULL	0	NULL	mood disorders	MedicalFinding		defined by					cognition	MentalProcess	presence of			NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar disorder or manic–depressive disorder, also referred to as bipolar affective disorder or manic depression, is a psychiatric diagnosis that describes a category of mood disorders defined by the presence of one or more episodes of abnormally elevated energy levels, cognition, and mood with or without one or more depressive episodes.	topic_bd
77882	8	356253	7	NULL	NULL	0	NULL	mood disorders	MedicalFinding		defined by					depressive episodes	MentalProcess	mood with			NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar disorder or manic–depressive disorder, also referred to as bipolar affective disorder or manic depression, is a psychiatric diagnosis that describes a category of mood disorders defined by the presence of one or more episodes of abnormally elevated energy levels, cognition, and mood with or without one or more depressive episodes.	topic_bd
77883	9	356253	7	NULL	NULL	0	NULL	mood disorders	MedicalFinding		defined by					depressive episodes	MedicalFinding	mood without			NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar disorder or manic–depressive disorder, also referred to as bipolar affective disorder or manic depression, is a psychiatric diagnosis that describes a category of mood disorders defined by the presence of one or more episodes of abnormally elevated energy levels, cognition, and mood with or without one or more depressive episodes.	topic_bd
77884	10	356253	7	NULL	NULL	0	NULL	statement 8	Process		is an alternative to					statement 9	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar disorder or manic–depressive disorder, also referred to as bipolar affective disorder or manic depression, is a psychiatric diagnosis that describes a category of mood disorders defined by the presence of one or more episodes of abnormally elevated energy levels, cognition, and mood with or without one or more depressive episodes.	topic_bd
77885	11	356253	7	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Bipolar disorder or manic–depressive disorder, also referred to as bipolar affective disorder or manic depression, is a psychiatric diagnosis that describes a category of mood disorders defined by the presence of one or more episodes of abnormally elevated energy levels, cognition, and mood with or without one or more depressive episodes.	topic_bd
77886	1	356254	7	NULL	NULL	0	NULL	Neurotransmitters	Chemical		is a type of					endogenous chemicals	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Neurotransmitters are endogenous chemicals that transmit signals from a neuron to a target cell across a synapse, and their dysfunction is associated with neurotransmitter diseases such as bipolar disorder.	topic_bd
77887	2	356254	7	NULL	NULL	NULL	NULL	neuron	Cell	signal from	transmitted to					target cell	Cell				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Neurotransmitters are endogenous chemicals that transmit signals from a neuron to a target cell across a synapse, and their dysfunction is associated with neurotransmitter diseases such as bipolar disorder.	topic_bd
77888	3	356254	7	NULL	NULL	0	NULL	statement 2	Process		via					synapse	CellComponent				NULL		0	NULL	NULL	NULL	NULL	NULL	Neurotransmitters are endogenous chemicals that transmit signals from a neuron to a target cell across a synapse, and their dysfunction is associated with neurotransmitter diseases such as bipolar disorder.	topic_bd
77889	4	356254	7	NULL	NULL	NULL	NULL	statement 3	Chemical	dysfunction of	associated with					bipolar disorder	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Neurotransmitters are endogenous chemicals that transmit signals from a neuron to a target cell across a synapse, and their dysfunction is associated with neurotransmitter diseases such as bipolar disorder.	topic_bd
77890	5	356254	7	NULL	NULL	0	NULL	bipolar disorder	MedicalFinding		is a type of					neurotransmitter disease	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Neurotransmitters are endogenous chemicals that transmit signals from a neuron to a target cell across a synapse, and their dysfunction is associated with neurotransmitter diseases such as bipolar disorder.	topic_bd
77891	1	356255	7	NULL	NULL	NULL	NULL	amygdala activation	Process	abnormal	is a state of					amygdala	OrganismPart	activity of above normal levels of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Abnormal amygdala activation is a state of activity of the amygdala above or below normal levels.	topic_bd
77892	2	356255	7	NULL	NULL	0	NULL	amygdala activation	Process	abnormal	is a state of					amygdala	OrganismPart	activity of below normal levels of			NULL		0	NULL	NULL	NULL	NULL	NULL	Abnormal amygdala activation is a state of activity of the amygdala above or below normal levels.	topic_bd
77893	1	356256	7	NULL	NULL	NULL	NULL	Memory loss	MentalProcess		decrease in					remember	MentalProcess	ability to			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Memory loss is the decrease in the ability to remember.	topic_bd
77894	1	356257	7	NULL	NULL	0	NULL	hypomania	MedicalFinding		is a type of					mood state	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Hypomania is a mood state characterized by persistent and pervasive elevated (euphoric) or irritable mood, as well as thoughts and behaviors that are consistent with such a mood state.	topic_bd
77895	2	356257	7	NULL	NULL	0	NULL	hypomania	MedicalFinding		characterized by					elevated mood	MentalProcess	persistent			NULL		0	NULL	NULL	NULL	NULL	NULL	Hypomania is a mood state characterized by persistent and pervasive elevated (euphoric) or irritable mood, as well as thoughts and behaviors that are consistent with such a mood state.	topic_bd
77896	3	356257	7	NULL	NULL	0	NULL	hypomania	MedicalFinding		characterized by					irritable mood	MentalProcess	persistent 			NULL		0	NULL	NULL	NULL	NULL	NULL	Hypomania is a mood state characterized by persistent and pervasive elevated (euphoric) or irritable mood, as well as thoughts and behaviors that are consistent with such a mood state.	topic_bd
77897	4	356257	7	NULL	NULL	0	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Hypomania is a mood state characterized by persistent and pervasive elevated (euphoric) or irritable mood, as well as thoughts and behaviors that are consistent with such a mood state.	topic_bd
77898	5	356257	7	NULL	NULL	0	NULL	hypomania	MedicalFinding		characterized by					elevated mood	MentalProcess	pervasive			NULL		0	NULL	NULL	NULL	NULL	NULL	Hypomania is a mood state characterized by persistent and pervasive elevated (euphoric) or irritable mood, as well as thoughts and behaviors that are consistent with such a mood state.	topic_bd
77899	6	356257	7	NULL	NULL	0	NULL	hypomania	MedicalFinding		characterized by					irritable mood	MentalProcess	pervasive			NULL		0	NULL	NULL	NULL	NULL	NULL	Hypomania is a mood state characterized by persistent and pervasive elevated (euphoric) or irritable mood, as well as thoughts and behaviors that are consistent with such a mood state.	topic_bd
77900	7	356257	7	NULL	NULL	0	NULL	statement 5	Process		is an alternative to					statement 6	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Hypomania is a mood state characterized by persistent and pervasive elevated (euphoric) or irritable mood, as well as thoughts and behaviors that are consistent with such a mood state.	topic_bd
77901	1	356258	7	NULL	NULL	0	NULL	abnormal brain structure	OrganismPart		deviates from					brain structure	OrganismPart	norm			NULL		0	NULL	NULL	NULL	NULL	NULL	An abnormal brain structure is a brain structure which deviates from the norm.	topic_bd
78426	1	356259	5	NULL	NULL	0	NULL	low-line animals	Organism		treated with					GLYX-13	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of low-line animals with the NMDAR glycine site partial agonist GLYX-13 rescued the deficits in play-induced pro-social 50-kHz and reduced monotonous USVs.	topic_aut
78427	2	356259	5	NULL	NULL	0	NULL	GLYX-13	Chemical		is a partial agonist of					NMDAR 	GP		glycine site		NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of low-line animals with the NMDAR glycine site partial agonist GLYX-13 rescued the deficits in play-induced pro-social 50-kHz and reduced monotonous USVs.	topic_aut
78428	3	356259	5	NULL	NULL	0	NULL	statement 1	Process		reduce					USVs	Process	monotonous			NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of low-line animals with the NMDAR glycine site partial agonist GLYX-13 rescued the deficits in play-induced pro-social 50-kHz and reduced monotonous USVs.	topic_aut
78429	1	356260	5	NULL	NULL	0	NULL	CNVs	NucleicAcid	multiple;;recurrent;; de novo	is associated with		strongly			autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple Recurrent De Novo CNVs, Including Duplications of the 7q11.23 Williams Syndrome Region, Are Strongly Associated with Autism.	topic_aut
78430	2	356260	5	NULL	NULL	0	NULL	CNVs	NucleicAcid	multiple;;recurrent;; de novo	include					7q11.23	Chromosome	duplications of			NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple Recurrent De Novo CNVs, Including Duplications of the 7q11.23 Williams Syndrome Region, Are Strongly Associated with Autism.	topic_aut
78431	3	356260	5	NULL	NULL	0	NULL	7q11.23	Chromosome		is					Williams Syndrome region	Chromosome				NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple Recurrent De Novo CNVs, Including Duplications of the 7q11.23 Williams Syndrome Region, Are Strongly Associated with Autism.	topic_aut
78432	1	356262	5	NULL	NULL	0	NULL	ARX gene	GP		cause					syndromic autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78433	2	356262	5	NULL	NULL	0	NULL	ARX gene	GP		cause					other cognitive disorders	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78434	3	356262	5	NULL	NULL	0	NULL	ATRX gene	GP		cause					syndromic autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78435	4	356262	5	NULL	NULL	0	NULL	ATRX gene	GP		cause					other cognitive disorders	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78436	5	356262	5	NULL	NULL	NULL	NULL	CACNA1C gene	GP		cause					syndromic autism	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78437	6	356262	5	NULL	NULL	0	NULL	CACNA1C gene	GP		cause					other cognitive disorders	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78438	7	356262	5	NULL	NULL	0	NULL	CDKL5 gene	GP		cause					syndromic autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78439	8	356262	5	NULL	NULL	0	NULL	CDKL5 gene	GP		cause					other cognitive disorders	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78440	9	356262	5	NULL	NULL	0	NULL	EML1 gene	GP		cause					syndromic autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78441	10	356262	5	NULL	NULL	0	NULL	EML1 gene	GP		cause					other cognitive disorders	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78442	11	356262	5	NULL	NULL	0	NULL	FMR1 gene	GP		cause					syndromic autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78443	12	356262	5	NULL	NULL	0	NULL	FMR1 gene	GP		cause					other cognitive disorders	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78444	13	356262	5	NULL	NULL	0	NULL	FOXP2 gene	GP		cause					syndromic autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78445	14	356262	5	NULL	NULL	0	NULL	FOXP2 gene	GP		cause					other cognitive disorders	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78446	15	356262	5	NULL	NULL	0	NULL	GRID2 gene	GP		cause					syndromic autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78447	16	356262	5	NULL	NULL	0	NULL	GRID2 gene	GP		cause					other cognitive disorders	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78448	17	356262	5	NULL	NULL	0	NULL	HOXA1 gene	GP		cause					syndromic autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78449	18	356262	5	NULL	NULL	0	NULL	HOXA1 gene	GP		cause					other cognitive disorders	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78450	19	356262	5	NULL	NULL	0	NULL	KCTD13 gene	GP		cause					syndromic autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78451	20	356262	5	NULL	NULL	0	NULL	KCTD13 gene	GP		cause					other cognitive disorders	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78452	21	356262	5	NULL	NULL	0	NULL	MAPK3 gene	GP		cause					syndromic autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78453	2	356262	5	NULL	NULL	NULL	NULL	MAPK3 gene	GP		cause					other cognitive disorders	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78454	22	356262	5	NULL	NULL	0	NULL	MAPK3 gene	GP		cause					other cognitive disorders	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78455	23	356262	5	NULL	NULL	0	NULL	MECP2 gene	GP		cause					syndromic autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78456	24	356262	5	NULL	NULL	0	NULL	MECP2 gene	GP		cause					other cognitive disorders	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78457	25	356262	5	NULL	NULL	0	NULL	NLGN3 gene	GP		cause					syndromic autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78458	26	356262	5	NULL	NULL	0	NULL	NLGN3 gene	GP		cause					other cognitive disorders	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78459	27	356262	5	NULL	NULL	0	NULL	NLGN4X gene	GP		cause					syndromic autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78460	28	356262	5	NULL	NULL	0	NULL	NLGN4X gene	GP		cause					other cognitive disorders	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78461	29	356262	5	NULL	NULL	0	NULL	PTEN gene	GP		cause					syndromic autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78462	30	356262	5	NULL	NULL	0	NULL	PTEN gene	GP		cause					other cognitive disorders	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78463	31	356262	5	NULL	NULL	0	NULL	RS1 gene	GP		cause					syndromic autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78464	32	356262	5	NULL	NULL	0	NULL	RS1 gene	GP		cause					other cognitive disorders	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78465	33	356262	5	NULL	NULL	0	NULL	SHANK3 gene	GP		cause					syndromic autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78466	34	356262	5	NULL	NULL	0	NULL	SHANK3 gene	GP		cause					other cognitive disorders	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78467	35	356262	5	NULL	NULL	0	NULL	SLC25A12 gene	GP		cause					syndromic autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78468	36	356262	5	NULL	NULL	0	NULL	SLC25A12 gene	GP		cause					other cognitive disorders	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78469	37	356262	5	NULL	NULL	0	NULL	TSC1 gene	GP		cause					syndromic autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78470	38	356262	5	NULL	NULL	0	NULL	TSC1 gene	GP		cause					other cognitive disorders	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78471	39	356262	5	NULL	NULL	0	NULL	TSC2 gene	GP		cause					syndromic autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78472	40	356262	5	NULL	NULL	0	NULL	TSC2 gene	GP		cause					other cognitive disorders	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78473	41	356262	5	NULL	NULL	0	NULL	UBE3A gene	GP		cause					syndromic autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
78474	42	356262	5	NULL	NULL	0	NULL	UBE3A gene	GP		cause					other cognitive disorders	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	We sequenced a total of 21 genes (ARX, ATRX, CACNA1C, CDKL5, EML1, FMR1, FOXP2, GRID2, HOXA1, KCTD13, MAPK3, MECP2, NLGN3, NLGN4X, PTEN, RS1, SHANK3, SLC25A12, TSC1, TSC2 and UBE3A) known to cause syndromic autism and other cognitive disorders	topic_aut
77902	1	356263	7	NULL	NULL	0	NULL	copper-64-diacetyl-bis (N4-methylthiosemicarbazone)	Chemical		reduces					tumorigenic cells	Cell	CD133+ highly			NULL		0	NULL	NULL	NULL	NULL	NULL	Internal radiotherapy with copper-64-diacetyl-bis (N4-methylthiosemicarbazone) reduces CD133+ highly tumorigenic cells and metastatic ability of mouse colon carcinoma.	topic_ccc
77903	2	356263	7	NULL	NULL	NULL	NULL	copper-64-diacetyl-bis (N4-methylthiosemicarbazone)	Chemical		reduces					 colon carcinoma	MedicalFinding	metastatic ability of mouse			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Internal radiotherapy with copper-64-diacetyl-bis (N4-methylthiosemicarbazone) reduces CD133+ highly tumorigenic cells and metastatic ability of mouse colon carcinoma.	topic_ccc
77904	1	356264	7	NULL	NULL	0	NULL	transgelin	GP		associate with					lymph node metastasis	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Association of the actin-binding protein transgelin with lymph node metastasis in human colorectal cancer.	topic_ccc
77905	2	356264	7	NULL	NULL	0	NULL	statement 1	Process		occur in					colorectal cancer	MedicalFinding	human			NULL		0	NULL	NULL	NULL	NULL	NULL	Association of the actin-binding protein transgelin with lymph node metastasis in human colorectal cancer.	topic_ccc
77906	3	356264	7	NULL	NULL	0	NULL	transgelin	GP		is a type of					actin-binding protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Association of the actin-binding protein transgelin with lymph node metastasis in human colorectal cancer.	topic_ccc
77907	1	356265	7	NULL	NULL	NULL	NULL	total dietary fat 	Food	intake of	associated with					colon cancer	MedicalFinding	risk of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	As with breast cancer, international comparisons initially suggested an association between total dietary fat intake and colon cancer risk.	topic_ccc
77908	1	356266	7	NULL	NULL	NULL	NULL	intratumoral regions	OrganismPart		shows					CD133(+) cells	Cell	high density of			NULL	mouse colon carcinoma (Colon-26) model	NULL	NULL	NULL	NULL	NULL	NULL	 In a mouse colon carcinoma (Colon-26) model, we have shown that (64)Cu-ATSM preferentially localizes in intratumoral regions with a high density of CD133(+) cells, which show characteristics of cancer stem cells or cancer stem cell-like cells (collectively referred here as CSCs).	topic_ccc
77909	2	356266	7	NULL	NULL	NULL	NULL	(64)Cu-ATSM	Chemical		localizes in		preferentially			statement 1	Process				NULL	mouse colon carcinoma (Colon-26) model	NULL	NULL	NULL	NULL	NULL	NULL	 In a mouse colon carcinoma (Colon-26) model, we have shown that (64)Cu-ATSM preferentially localizes in intratumoral regions with a high density of CD133(+) cells, which show characteristics of cancer stem cells or cancer stem cell-like cells (collectively referred here as CSCs).	topic_ccc
77910	3	356266	7	NULL	NULL	NULL	NULL	CD133(+) cells	Cell		shows					cancer stem cells	Cell	characteristics of			NULL	mouse colon carcinoma (Colon-26) model	NULL	NULL	NULL	NULL	NULL	NULL	 In a mouse colon carcinoma (Colon-26) model, we have shown that (64)Cu-ATSM preferentially localizes in intratumoral regions with a high density of CD133(+) cells, which show characteristics of cancer stem cells or cancer stem cell-like cells (collectively referred here as CSCs).	topic_ccc
77911	4	356266	7	NULL	NULL	NULL	NULL	CD133(+) cells	Cell		shows					CSCs	Cell	characteristics of			NULL	mouse colon carcinoma (Colon-26) model	NULL	NULL	NULL	NULL	NULL	NULL	 In a mouse colon carcinoma (Colon-26) model, we have shown that (64)Cu-ATSM preferentially localizes in intratumoral regions with a high density of CD133(+) cells, which show characteristics of cancer stem cells or cancer stem cell-like cells (collectively referred here as CSCs).	topic_ccc
77912	5	356266	7	NULL	NULL	NULL	NULL	CSCs	Cell		is					cancer stem cell-like cells 	Cell				NULL	mouse colon carcinoma (Colon-26) model	NULL	NULL	NULL	NULL	NULL	NULL	 In a mouse colon carcinoma (Colon-26) model, we have shown that (64)Cu-ATSM preferentially localizes in intratumoral regions with a high density of CD133(+) cells, which show characteristics of cancer stem cells or cancer stem cell-like cells (collectively referred here as CSCs).	topic_ccc
77913	1	356268	7	NULL	NULL	0	NULL	64)Cu-ATSM	Chemical		inhibit					tumor growth	Process				NULL	in vivo	0	NULL	NULL	NULL	NULL	NULL	In vivo studies showed that (64)Cu-ATSM treatment inhibited tumor growth. The percentage of CD133(+) cells and metastatic ability in (64)Cu-ATSM treated tumors was decreased compared with that in control animals.	topic_ccc
77914	1	356269	7	NULL	NULL	NULL	NULL	(64)Cu-ATSM	Chemical		accumulates in					cells	Cell				NULL	in vitro	NULL	NULL	NULL	NULL	NULL	NULL	 In vitro studies demonstrated that (64)Cu-ATSM accumulated in cells under hypoxic conditions and incorporation of (64)Cu-ATSM under hypoxia caused cell death in both CD133(+) and CD133(-) cells in a similar extent.	topic_ccc
77915	2	356269	7	NULL	NULL	0	NULL	statement 1	Process		occur under					hypoxic condition	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 In vitro studies demonstrated that (64)Cu-ATSM accumulated in cells under hypoxic conditions and incorporation of (64)Cu-ATSM under hypoxia caused cell death in both CD133(+) and CD133(-) cells in a similar extent.	topic_ccc
77916	3	356269	7	NULL	NULL	NULL	NULL	statement 2	Process		cause					 CD133(+) cells	Cell	cell death of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	 In vitro studies demonstrated that (64)Cu-ATSM accumulated in cells under hypoxic conditions and incorporation of (64)Cu-ATSM under hypoxia caused cell death in both CD133(+) and CD133(-) cells in a similar extent.	topic_ccc
77917	4	356269	7	NULL	NULL	0	NULL	statement 2	Process		cause					CD133(-) cells	Cell	cell death of			NULL		0	NULL	NULL	NULL	NULL	NULL	 In vitro studies demonstrated that (64)Cu-ATSM accumulated in cells under hypoxic conditions and incorporation of (64)Cu-ATSM under hypoxia caused cell death in both CD133(+) and CD133(-) cells in a similar extent.	topic_ccc
77918	5	356269	7	NULL	NULL	0	NULL	statement 3	Process		is similar to					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 In vitro studies demonstrated that (64)Cu-ATSM accumulated in cells under hypoxic conditions and incorporation of (64)Cu-ATSM under hypoxia caused cell death in both CD133(+) and CD133(-) cells in a similar extent.	topic_ccc
77919	1	356270	7	NULL	NULL	0	NULL	Cu-ATSM	Chemical		reduce					tumor	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Cu-ATSM administration reduced tumor volume as well as the percentage of CD133(+) cells and the metastatic ability of Colon-26 tumors.	topic_ccc
77920	2	356270	7	NULL	NULL	0	NULL	Cu-ATSM	Chemical		reduce					CD133(+) cells	Cell	percentage of			NULL		0	NULL	NULL	NULL	NULL	NULL	Cu-ATSM administration reduced tumor volume as well as the percentage of CD133(+) cells and the metastatic ability of Colon-26 tumors.	topic_ccc
77921	3	356270	7	NULL	NULL	0	NULL	Cu-ATSM	Chemical		reduce					Colon-26 tumors	MedicalFinding	metastatic ability of			NULL		0	NULL	NULL	NULL	NULL	NULL	Cu-ATSM administration reduced tumor volume as well as the percentage of CD133(+) cells and the metastatic ability of Colon-26 tumors.	topic_ccc
77922	1	356271	7	NULL	NULL	NULL	NULL	MZF	Chemical		upregulate					CD80	Cell	expression of			NULL	bone marrow DCs	NULL	NULL	NULL	NULL	NULL	NULL	In this study, we demonstrated that MZF upregulated the expression of CD80, CD86, CD83, and MHC II on bone marrow-derived dendritic cells (DCs) and significantly increased interleukin-12 (IL-12) and tumor necrosis factor-alpha production by DCs in a dose-dependent manner.	topic_ccc
77923	2	356271	7	NULL	NULL	NULL	NULL	MZF	Chemical		upregulate					CD86	Cell	expression of			NULL	bone marrow DCs	NULL	NULL	NULL	NULL	NULL	NULL	In this study, we demonstrated that MZF upregulated the expression of CD80, CD86, CD83, and MHC II on bone marrow-derived dendritic cells (DCs) and significantly increased interleukin-12 (IL-12) and tumor necrosis factor-alpha production by DCs in a dose-dependent manner.	topic_ccc
77924	3	356271	7	NULL	NULL	NULL	NULL	MZF	Chemical		upregulate					CD83	Cell	expression of			NULL	bone marrow DCs	NULL	NULL	NULL	NULL	NULL	NULL	In this study, we demonstrated that MZF upregulated the expression of CD80, CD86, CD83, and MHC II on bone marrow-derived dendritic cells (DCs) and significantly increased interleukin-12 (IL-12) and tumor necrosis factor-alpha production by DCs in a dose-dependent manner.	topic_ccc
77925	4	356271	7	NULL	NULL	NULL	NULL	MZF	Chemical		upregulate					MHC II	Cell	expression of			NULL	bone marrow DCs	NULL	NULL	NULL	NULL	NULL	NULL	In this study, we demonstrated that MZF upregulated the expression of CD80, CD86, CD83, and MHC II on bone marrow-derived dendritic cells (DCs) and significantly increased interleukin-12 (IL-12) and tumor necrosis factor-alpha production by DCs in a dose-dependent manner.	topic_ccc
77926	5	356271	7	NULL	NULL	0	NULL	bone marrow DCs	Cell		is					bone marrow-derived dendritic cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	In this study, we demonstrated that MZF upregulated the expression of CD80, CD86, CD83, and MHC II on bone marrow-derived dendritic cells (DCs) and significantly increased interleukin-12 (IL-12) and tumor necrosis factor-alpha production by DCs in a dose-dependent manner.	topic_ccc
77927	6	356271	7	NULL	NULL	0	NULL	DCs	Cell		produce					IL-12	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	In this study, we demonstrated that MZF upregulated the expression of CD80, CD86, CD83, and MHC II on bone marrow-derived dendritic cells (DCs) and significantly increased interleukin-12 (IL-12) and tumor necrosis factor-alpha production by DCs in a dose-dependent manner.	topic_ccc
77928	7	356271	7	NULL	NULL	NULL	NULL	DCs	Cell		produce					tumor necrosis factor-alpha	GP				NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study, we demonstrated that MZF upregulated the expression of CD80, CD86, CD83, and MHC II on bone marrow-derived dendritic cells (DCs) and significantly increased interleukin-12 (IL-12) and tumor necrosis factor-alpha production by DCs in a dose-dependent manner.	topic_ccc
77929	8	356271	7	NULL	NULL	0	NULL	MZF	Chemical		increase		dose-dependently;;significantly			statement 6	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	In this study, we demonstrated that MZF upregulated the expression of CD80, CD86, CD83, and MHC II on bone marrow-derived dendritic cells (DCs) and significantly increased interleukin-12 (IL-12) and tumor necrosis factor-alpha production by DCs in a dose-dependent manner.	topic_ccc
77930	9	356271	7	NULL	NULL	0	NULL	MZF	Chemical		increase		dose-dependently;;significantly			statement 7	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	In this study, we demonstrated that MZF upregulated the expression of CD80, CD86, CD83, and MHC II on bone marrow-derived dendritic cells (DCs) and significantly increased interleukin-12 (IL-12) and tumor necrosis factor-alpha production by DCs in a dose-dependent manner.	topic_ccc
77931	10	356271	7	NULL	NULL	0	NULL	IL-12	GP		is					interleukin-12	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	In this study, we demonstrated that MZF upregulated the expression of CD80, CD86, CD83, and MHC II on bone marrow-derived dendritic cells (DCs) and significantly increased interleukin-12 (IL-12) and tumor necrosis factor-alpha production by DCs in a dose-dependent manner.	topic_ccc
77932	1	356273	7	NULL	NULL	0	NULL	GH1 gene	GP		encode					somatotropin	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Somatotropin is a protein that in humans is encoded by the GH1 gene.	topic_ccc
77933	2	356273	7	NULL	NULL	0	NULL	statement 1	Process		occur in					human	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Somatotropin is a protein that in humans is encoded by the GH1 gene.	topic_ccc
77934	1	356274	7	NULL	NULL	0	NULL	Growth Factor	GP		functions to					cell division	Process	regulate			NULL		0	NULL	NULL	NULL	NULL	NULL	Growth Factor is a protein molecule made by the body; it functions to regulate cell division & cell survival.	topic_ccc
77935	2	356274	7	NULL	NULL	0	NULL	Growth Factor	GP		functions to					cell survival	Process	regulate			NULL		0	NULL	NULL	NULL	NULL	NULL	Growth Factor is a protein molecule made by the body; it functions to regulate cell division & cell survival.	topic_ccc
77936	3	356274	7	NULL	NULL	0	NULL	Growth Factor	GP		is a type of					protein molecule	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Growth Factor is a protein molecule made by the body; it functions to regulate cell division & cell survival.	topic_ccc
77937	1	356275	7	NULL	NULL	0	NULL	alpha-defensin	GP	expression of	is enhanced in					colon cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	It is known that alpha-defensin expression is enhanced in colon cancer. 	topic_ccc
77938	1	356276	7	NULL	NULL	0	NULL	MZF	Chemical		inhibit		significantly			tumor growth	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	We previously isolated the novel heteropolysaccharide maitake Z-fraction (MZF) from the maitake mushroom (Grifola frondosa), and demonstrated that MZF significantly inhibited tumor growth by inducing cell-mediated immunity.	topic_ccc
77939	2	356276	7	NULL	NULL	0	NULL	statement 1	Process		occur by					cell-mediated immunity	Process	inducing			NULL		0	NULL	NULL	NULL	NULL	NULL	We previously isolated the novel heteropolysaccharide maitake Z-fraction (MZF) from the maitake mushroom (Grifola frondosa), and demonstrated that MZF significantly inhibited tumor growth by inducing cell-mediated immunity.	topic_ccc
77940	3	356276	7	NULL	NULL	0	NULL	MZF	Chemical		is					maitake Z-fraction	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	We previously isolated the novel heteropolysaccharide maitake Z-fraction (MZF) from the maitake mushroom (Grifola frondosa), and demonstrated that MZF significantly inhibited tumor growth by inducing cell-mediated immunity.	topic_ccc
77941	4	356276	7	NULL	NULL	0	NULL	MZF	Chemical		is a type of					novel heteropolysaccharide	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	We previously isolated the novel heteropolysaccharide maitake Z-fraction (MZF) from the maitake mushroom (Grifola frondosa), and demonstrated that MZF significantly inhibited tumor growth by inducing cell-mediated immunity.	topic_ccc
77942	5	356276	7	NULL	NULL	0	NULL	MZF	Chemical		obtained from					maitake mushroom 	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	We previously isolated the novel heteropolysaccharide maitake Z-fraction (MZF) from the maitake mushroom (Grifola frondosa), and demonstrated that MZF significantly inhibited tumor growth by inducing cell-mediated immunity.	topic_ccc
77944	6	356276	7	NULL	NULL	0	NULL	maitake mushroom	Organism		is					Grifola frondosa	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	We previously isolated the novel heteropolysaccharide maitake Z-fraction (MZF) from the maitake mushroom (Grifola frondosa), and demonstrated that MZF significantly inhibited tumor growth by inducing cell-mediated immunity.	topic_ccc
78504	1	356277	5	NULL	NULL	0	NULL	FC	GroupOfPeople		is predisposed to					autism spectrum disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Our initial analysis revealed the presence of association at two loci: DXS6789 (P=0.026) and DXS8043 (P=0.0101). In a second step, we added support to the association at DXS8043 using additional markers, additional subjects and a haplotype-based analysis (best obtained P-value=0.00001). These results provide support for the existence of a locus on the X chromosome that predisposes the FC to autism spectrum disorders.	topic_aut
78508	2	356277	5	NULL	NULL	0	NULL	X chromosome	Chromosome		plays a role in					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Our initial analysis revealed the presence of association at two loci: DXS6789 (P=0.026) and DXS8043 (P=0.0101). In a second step, we added support to the association at DXS8043 using additional markers, additional subjects and a haplotype-based analysis (best obtained P-value=0.00001). These results provide support for the existence of a locus on the X chromosome that predisposes the FC to autism spectrum disorders.	topic_aut
78510	1	356278	5	NULL	NULL	0	NULL	ARX	GP		is					Aristaless related homeobox	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Aristaless related homeobox (ARX) is a paired-type homeobox gene	topic_aut
78511	2	356278	5	NULL	NULL	0	NULL	ARX gene	GP		is a type of					paired-type homeobox gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Aristaless related homeobox (ARX) is a paired-type homeobox gene	topic_aut
78518	1	356280	5	NULL	NULL	0	NULL	cyclin-dependent kinase-like 5	GP		is also known as					STK9	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	CDKL5 is a gene that provides instructions for making a protein called cyclin-dependent kinase-like 5 also known as serine/threonine kinase 9 (STK9)	topic_aut
78519	2	356280	5	NULL	NULL	0	NULL	STK9	GP		is					serine/threonine kinase 9	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	CDKL5 is a gene that provides instructions for making a protein called cyclin-dependent kinase-like 5 also known as serine/threonine kinase 9 (STK9)	topic_aut
78520	3	356280	5	NULL	NULL	0	NULL	CDKL5 gene	GP		encodes for					cyclin-dependent kinase-like 5 protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	CDKL5 is a gene that provides instructions for making a protein called cyclin-dependent kinase-like 5 also known as serine/threonine kinase 9 (STK9)	topic_aut
78521	1	356281	5	NULL	NULL	NULL	NULL	Echinoderm microtubule-associated protein-like 1 protein	GP	human	is encoded by					EML1 gene	GP	human			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Echinoderm microtubule-associated protein-like 1 is a protein that in humans is encoded by the EML1 gene	topic_aut
78522	1	356283	5	NULL	NULL	0	NULL	Forkhead box protein P2	GP		is also known as					FOXP2	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Forkhead box protein P2 also known as FOXP2 is a protein that in humans is encoded by the FOXP2 gene	topic_aut
78523	2	356283	5	NULL	NULL	0	NULL	FOXP2 protein	GP	human	is encoded by					FOXP2 gene	GP	human			NULL		0	NULL	NULL	NULL	NULL	NULL	Forkhead box protein P2 also known as FOXP2 is a protein that in humans is encoded by the FOXP2 gene	topic_aut
78524	1	356288	5	NULL	NULL	0	NULL	PTEN	GP		is					Phosphatase and tensin homolog	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphatase and tensin homolog (PTEN) is a protein that, in humans, is encoded by the PTEN gene	topic_aut
78525	2	356288	5	NULL	NULL	0	NULL	PTEN protein	GP	human	is encoded by					PTEN gene	GP	human			NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphatase and tensin homolog (PTEN) is a protein that, in humans, is encoded by the PTEN gene	topic_aut
78526	1	356289	5	NULL	NULL	0	NULL	Retinoschisin	GP		is also known as					X-linked juvenile retinoschisis protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Retinoschisin also known as X-linked juvenile retinoschisis protein is a protein that in humans is encoded by the RS1 gene	topic_aut
78527	2	356289	5	NULL	NULL	0	NULL	X-linked juvenile retinoschisis protein	GP	human	is encoded by					RS1 gene	GP	human			NULL		0	NULL	NULL	NULL	NULL	NULL	Retinoschisin also known as X-linked juvenile retinoschisis protein is a protein that in humans is encoded by the RS1 gene	topic_aut
78528	1	356294	5	NULL	NULL	0	NULL	homocysteine	AminoAcid	plasma	elevated in		significantly			autism mothers	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic profiling indicated that plasma homocysteine, adenosine, and S-adenosylhomocyteine were significantly elevated among autism mothers consistent with reduced methylation capacity and DNA hypomethylation. Together, these results suggest that the maternal genetics/epigenetics may influence fetal predisposition to autism.	topic_aut
78529	2	356294	5	NULL	NULL	0	NULL	adenosine	NucleicAcid		elevated in		significantly			autism mothers	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic profiling indicated that plasma homocysteine, adenosine, and S-adenosylhomocyteine were significantly elevated among autism mothers consistent with reduced methylation capacity and DNA hypomethylation. Together, these results suggest that the maternal genetics/epigenetics may influence fetal predisposition to autism.	topic_aut
78530	3	356294	5	NULL	NULL	0	NULL	S-adenosylhomocyteine	AminoAcid		elevated in		significantly			autism mothers	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic profiling indicated that plasma homocysteine, adenosine, and S-adenosylhomocyteine were significantly elevated among autism mothers consistent with reduced methylation capacity and DNA hypomethylation. Together, these results suggest that the maternal genetics/epigenetics may influence fetal predisposition to autism.	topic_aut
78531	4	356294	5	NULL	NULL	0	NULL	methylation capacity	Process		reduced in					autism mothers	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic profiling indicated that plasma homocysteine, adenosine, and S-adenosylhomocyteine were significantly elevated among autism mothers consistent with reduced methylation capacity and DNA hypomethylation. Together, these results suggest that the maternal genetics/epigenetics may influence fetal predisposition to autism.	topic_aut
78532	5	356294	5	NULL	NULL	0	NULL	DNA hypomethylation	Process		reduced in					autism mothers	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic profiling indicated that plasma homocysteine, adenosine, and S-adenosylhomocyteine were significantly elevated among autism mothers consistent with reduced methylation capacity and DNA hypomethylation. Together, these results suggest that the maternal genetics/epigenetics may influence fetal predisposition to autism.	topic_aut
78533	6	356294	5	NULL	NULL	0	NULL	maternal genetics	Process		is also known as					epigenetics	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic profiling indicated that plasma homocysteine, adenosine, and S-adenosylhomocyteine were significantly elevated among autism mothers consistent with reduced methylation capacity and DNA hypomethylation. Together, these results suggest that the maternal genetics/epigenetics may influence fetal predisposition to autism.	topic_aut
78534	7	356294	5	NULL	NULL	0	NULL	epigenetics	Process		influence					autism	MedicalFinding	predisposition of;;fetal			NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic profiling indicated that plasma homocysteine, adenosine, and S-adenosylhomocyteine were significantly elevated among autism mothers consistent with reduced methylation capacity and DNA hypomethylation. Together, these results suggest that the maternal genetics/epigenetics may influence fetal predisposition to autism.	topic_aut
78535	1	356295	5	NULL	NULL	NULL	NULL	MECP2	GP		methylated in				promoter	autism male	GroupOfPeople	frontal cortex of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	A more frequent occurrence was significantly increased MECP2 promoter methylation in autism male frontal cortex compared to controls.	topic_aut
78536	2	356295	5	NULL	NULL	NULL	NULL	MECP2	GP		methylated in				promoter	controls	GroupOfPeople				NULL		NULL	NULL	NULL	NULL	NULL	NULL	A more frequent occurrence was significantly increased MECP2 promoter methylation in autism male frontal cortex compared to controls.	topic_aut
78537	3	356295	5	NULL	NULL	0	NULL	statement 1	Process		is increased than		significantly			statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	A more frequent occurrence was significantly increased MECP2 promoter methylation in autism male frontal cortex compared to controls.	topic_aut
78538	1	356296	5	NULL	NULL	0	NULL	genetic defects	MedicalFinding		reduce					MeCP2	GP	expression of			NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore, percent promoter methylation of MECP2 significantly correlated with reduced MeCP2 protein expression. These results suggest that both genetic and epigenetic defects lead to reduced MeCP2 expression and may be important in the complex etiology of autism.	topic_aut
78539	2	356296	5	NULL	NULL	0	NULL	epigenetic defects	MedicalFinding		reduce					MeCP2	GP	expression of			NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore, percent promoter methylation of MECP2 significantly correlated with reduced MeCP2 protein expression. These results suggest that both genetic and epigenetic defects lead to reduced MeCP2 expression and may be important in the complex etiology of autism.	topic_aut
78540	3	356296	5	NULL	NULL	0	NULL	statement 1	Process		plays a role in		may;;important			autism	MedicalFinding	complex etiology of			NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore, percent promoter methylation of MECP2 significantly correlated with reduced MeCP2 protein expression. These results suggest that both genetic and epigenetic defects lead to reduced MeCP2 expression and may be important in the complex etiology of autism.	topic_aut
78541	4	356296	5	NULL	NULL	0	NULL	statement 2	Process		plays a role in					autism	MedicalFinding	complex etiology of			NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore, percent promoter methylation of MECP2 significantly correlated with reduced MeCP2 protein expression. These results suggest that both genetic and epigenetic defects lead to reduced MeCP2 expression and may be important in the complex etiology of autism.	topic_aut
78542	1	356298	5	NULL	NULL	0	NULL	NRXN1 gene	GP		is vulnerable to					SCZ	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings demonstrate that the NRXN1 gene, a vulnerability gene for SCZ and ASD, influences brain structure and cognitive function susceptible in both disorders	topic_aut
78543	2	356298	5	NULL	NULL	0	NULL	NRXN1 gene	GP		is vulnerable to					ASD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings demonstrate that the NRXN1 gene, a vulnerability gene for SCZ and ASD, influences brain structure and cognitive function susceptible in both disorders	topic_aut
78544	3	356298	5	NULL	NULL	0	NULL	NRXN1 gene	GP		influence					brain structure	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings demonstrate that the NRXN1 gene, a vulnerability gene for SCZ and ASD, influences brain structure and cognitive function susceptible in both disorders	topic_aut
78545	4	356298	5	NULL	NULL	0	NULL	statement 2	Process		influence					cognitive functions	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings demonstrate that the NRXN1 gene, a vulnerability gene for SCZ and ASD, influences brain structure and cognitive function susceptible in both disorders	topic_aut
80654	1	356299	5	NULL	NULL	0	NULL	DRB1	Gene	allelic variation of	modulates		pleiotropically			rheumatoid arthritis	Disease	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	These data allow robust testing of the hypotheses that allelic variation at DRB1 pleiotropically modulates risk of rheumatoid arthritis, autism and schizophrenia. Systematic review of the literature indicates that reported associations of DRB1 variants with these three conditions are congruent with a pleiotropic model: DRB1*04 alleles have been associated with increased risk of rheumatoid arthritis and autism but decreased risk of schizophrenia, and DRB1*13 alleles have been associated with protection from rheumatoid arthritis and autism but higher risk of schizophrenia.	topic_aut
80655	2	356299	5	NULL	NULL	0	NULL	DRB1	Gene	allelic variation of	modulates		pleiotropically			autism	Disease	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	These data allow robust testing of the hypotheses that allelic variation at DRB1 pleiotropically modulates risk of rheumatoid arthritis, autism and schizophrenia. Systematic review of the literature indicates that reported associations of DRB1 variants with these three conditions are congruent with a pleiotropic model: DRB1*04 alleles have been associated with increased risk of rheumatoid arthritis and autism but decreased risk of schizophrenia, and DRB1*13 alleles have been associated with protection from rheumatoid arthritis and autism but higher risk of schizophrenia.	topic_aut
80656	3	356299	5	NULL	NULL	NULL	NULL	DRB1	Gene	allelic variation of	modulates		pleiotropically			schizophrenia	Disease	risk of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data allow robust testing of the hypotheses that allelic variation at DRB1 pleiotropically modulates risk of rheumatoid arthritis, autism and schizophrenia. Systematic review of the literature indicates that reported associations of DRB1 variants with these three conditions are congruent with a pleiotropic model: DRB1*04 alleles have been associated with increased risk of rheumatoid arthritis and autism but decreased risk of schizophrenia, and DRB1*13 alleles have been associated with protection from rheumatoid arthritis and autism but higher risk of schizophrenia.	topic_aut
80657	4	356299	5	NULL	NULL	0	NULL	DRB1*04 alleles	Gene		is associated with					rheumatoid arthritis	Disease	increased risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	These data allow robust testing of the hypotheses that allelic variation at DRB1 pleiotropically modulates risk of rheumatoid arthritis, autism and schizophrenia. Systematic review of the literature indicates that reported associations of DRB1 variants with these three conditions are congruent with a pleiotropic model: DRB1*04 alleles have been associated with increased risk of rheumatoid arthritis and autism but decreased risk of schizophrenia, and DRB1*13 alleles have been associated with protection from rheumatoid arthritis and autism but higher risk of schizophrenia.	topic_aut
80658	5	356299	5	NULL	NULL	0	NULL	DRB1*04 alleles	Gene		is associated with					autism	Disease	increased risk for			NULL		0	NULL	NULL	NULL	NULL	NULL	These data allow robust testing of the hypotheses that allelic variation at DRB1 pleiotropically modulates risk of rheumatoid arthritis, autism and schizophrenia. Systematic review of the literature indicates that reported associations of DRB1 variants with these three conditions are congruent with a pleiotropic model: DRB1*04 alleles have been associated with increased risk of rheumatoid arthritis and autism but decreased risk of schizophrenia, and DRB1*13 alleles have been associated with protection from rheumatoid arthritis and autism but higher risk of schizophrenia.	topic_aut
80659	6	356299	5	NULL	NULL	0	NULL	DRB1*04 alleles	Gene		is associated with					schizophrenia	Disease	decreased risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	These data allow robust testing of the hypotheses that allelic variation at DRB1 pleiotropically modulates risk of rheumatoid arthritis, autism and schizophrenia. Systematic review of the literature indicates that reported associations of DRB1 variants with these three conditions are congruent with a pleiotropic model: DRB1*04 alleles have been associated with increased risk of rheumatoid arthritis and autism but decreased risk of schizophrenia, and DRB1*13 alleles have been associated with protection from rheumatoid arthritis and autism but higher risk of schizophrenia.	topic_aut
80660	7	356299	5	NULL	NULL	0	NULL	DRB1*13 alleles	Gene		is associated with					rheumatoid arthritis	Disease	protection from			NULL		0	NULL	NULL	NULL	NULL	NULL	These data allow robust testing of the hypotheses that allelic variation at DRB1 pleiotropically modulates risk of rheumatoid arthritis, autism and schizophrenia. Systematic review of the literature indicates that reported associations of DRB1 variants with these three conditions are congruent with a pleiotropic model: DRB1*04 alleles have been associated with increased risk of rheumatoid arthritis and autism but decreased risk of schizophrenia, and DRB1*13 alleles have been associated with protection from rheumatoid arthritis and autism but higher risk of schizophrenia.	topic_aut
80661	8	356299	5	NULL	NULL	0	NULL	DRB1*13 alleles	Gene		is associated with					autism	Disease	protection from			NULL		0	NULL	NULL	NULL	NULL	NULL	These data allow robust testing of the hypotheses that allelic variation at DRB1 pleiotropically modulates risk of rheumatoid arthritis, autism and schizophrenia. Systematic review of the literature indicates that reported associations of DRB1 variants with these three conditions are congruent with a pleiotropic model: DRB1*04 alleles have been associated with increased risk of rheumatoid arthritis and autism but decreased risk of schizophrenia, and DRB1*13 alleles have been associated with protection from rheumatoid arthritis and autism but higher risk of schizophrenia.	topic_aut
80663	9	356299	5	NULL	NULL	0	NULL	DRB1*13 alleles	Gene		is associated with					schizophrenia	Disease	higher risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	These data allow robust testing of the hypotheses that allelic variation at DRB1 pleiotropically modulates risk of rheumatoid arthritis, autism and schizophrenia. Systematic review of the literature indicates that reported associations of DRB1 variants with these three conditions are congruent with a pleiotropic model: DRB1*04 alleles have been associated with increased risk of rheumatoid arthritis and autism but decreased risk of schizophrenia, and DRB1*13 alleles have been associated with protection from rheumatoid arthritis and autism but higher risk of schizophrenia.	topic_aut
78546	1	356302	5	NULL	NULL	0	NULL	SHANK3	GP		is mutated in					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	SHANK3 mutations identified in autism lead to modification of dendritic spine morphology via an actin-dependent mechanism.	topic_aut
78547	2	356302	5	NULL	NULL	0	NULL	SHANK3	GP	mutation of	modifies					dendritic spine morphology	PhysicalPhenomenon				NULL		0	NULL	NULL	NULL	NULL	NULL	SHANK3 mutations identified in autism lead to modification of dendritic spine morphology via an actin-dependent mechanism.	topic_aut
78548	3	356302	5	NULL	NULL	0	NULL	statement 2	Process		via					actin-dependent mechanism	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	SHANK3 mutations identified in autism lead to modification of dendritic spine morphology via an actin-dependent mechanism.	topic_aut
78639	1	356303	5	NULL	NULL	NULL	NULL	Shank3	Protein		plays a role in					spine induction	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	The de novo mutation in the ankyrin domain (Q321R) modifies the roles of Shank3 in spine induction and morphology, and actin accumulation in spines and affects growth cone motility. Finally, the two inherited mutations (R12C and R300C) have intermediate effects on spine density and synaptic transmission. Therefore, although inherited by healthy parents, the functional effects of these mutations strongly suggest that they could represent risk factors for ASD	topic_aut
78640	2	356303	5	NULL	NULL	NULL	NULL	Shank3	Protein		plays a role in					morphology	PhysicalPhenomenon				NULL		NULL	NULL	NULL	NULL	NULL	NULL	The de novo mutation in the ankyrin domain (Q321R) modifies the roles of Shank3 in spine induction and morphology, and actin accumulation in spines and affects growth cone motility. Finally, the two inherited mutations (R12C and R300C) have intermediate effects on spine density and synaptic transmission. Therefore, although inherited by healthy parents, the functional effects of these mutations strongly suggest that they could represent risk factors for ASD	topic_aut
80665	3	356303	5	NULL	NULL	0	NULL	actin	Protein		accumulates in					spine	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	The de novo mutation in the ankyrin domain (Q321R) modifies the roles of Shank3 in spine induction and morphology, and actin accumulation in spines and affects growth cone motility. Finally, the two inherited mutations (R12C and R300C) have intermediate effects on spine density and synaptic transmission. Therefore, although inherited by healthy parents, the functional effects of these mutations strongly suggest that they could represent risk factors for ASD	topic_aut
80669	4	356303	5	NULL	NULL	0	NULL	Shank3	Protein	de novo mutation of	modifies			ankyrin domain (Q321R)		statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The de novo mutation in the ankyrin domain (Q321R) modifies the roles of Shank3 in spine induction and morphology, and actin accumulation in spines and affects growth cone motility. Finally, the two inherited mutations (R12C and R300C) have intermediate effects on spine density and synaptic transmission. Therefore, although inherited by healthy parents, the functional effects of these mutations strongly suggest that they could represent risk factors for ASD	topic_aut
80670	5	356303	5	NULL	NULL	0	NULL	Shank3	Protein	de novo mutation of	modifies			ankyrin domain (Q321R)		statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The de novo mutation in the ankyrin domain (Q321R) modifies the roles of Shank3 in spine induction and morphology, and actin accumulation in spines and affects growth cone motility. Finally, the two inherited mutations (R12C and R300C) have intermediate effects on spine density and synaptic transmission. Therefore, although inherited by healthy parents, the functional effects of these mutations strongly suggest that they could represent risk factors for ASD	topic_aut
80672	6	356303	5	NULL	NULL	0	NULL	Shank3	Protein	de novo mutation of	modifies			ankyrin domain (Q321R)		statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The de novo mutation in the ankyrin domain (Q321R) modifies the roles of Shank3 in spine induction and morphology, and actin accumulation in spines and affects growth cone motility. Finally, the two inherited mutations (R12C and R300C) have intermediate effects on spine density and synaptic transmission. Therefore, although inherited by healthy parents, the functional effects of these mutations strongly suggest that they could represent risk factors for ASD	topic_aut
80673	6	356303	5	NULL	NULL	0	NULL	Shank3	Protein	de novo mutation of	modifies			ankyrin domain (Q321R)		statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The de novo mutation in the ankyrin domain (Q321R) modifies the roles of Shank3 in spine induction and morphology, and actin accumulation in spines and affects growth cone motility. Finally, the two inherited mutations (R12C and R300C) have intermediate effects on spine density and synaptic transmission. Therefore, although inherited by healthy parents, the functional effects of these mutations strongly suggest that they could represent risk factors for ASD	topic_aut
80676	7	356303	5	NULL	NULL	0	NULL	Shank3	Protein	de novo mutation of	affects			ankyrin domain (Q321R)		growth cone motility	BiologicalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	The de novo mutation in the ankyrin domain (Q321R) modifies the roles of Shank3 in spine induction and morphology, and actin accumulation in spines and affects growth cone motility. Finally, the two inherited mutations (R12C and R300C) have intermediate effects on spine density and synaptic transmission. Therefore, although inherited by healthy parents, the functional effects of these mutations strongly suggest that they could represent risk factors for ASD	topic_aut
80679	8	356303	5	NULL	NULL	0	NULL	R12C	AminoAcid		is a type of					inherited mutations	AminoAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	The de novo mutation in the ankyrin domain (Q321R) modifies the roles of Shank3 in spine induction and morphology, and actin accumulation in spines and affects growth cone motility. Finally, the two inherited mutations (R12C and R300C) have intermediate effects on spine density and synaptic transmission. Therefore, although inherited by healthy parents, the functional effects of these mutations strongly suggest that they could represent risk factors for ASD	topic_aut
80680	9	356303	5	NULL	NULL	0	NULL	R300C	AminoAcid		is a type of					inherited mutations	AminoAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	The de novo mutation in the ankyrin domain (Q321R) modifies the roles of Shank3 in spine induction and morphology, and actin accumulation in spines and affects growth cone motility. Finally, the two inherited mutations (R12C and R300C) have intermediate effects on spine density and synaptic transmission. Therefore, although inherited by healthy parents, the functional effects of these mutations strongly suggest that they could represent risk factors for ASD	topic_aut
78549	1	356304	5	NULL	NULL	0	NULL	DISC1	GP		plays a role in		may			autism	MedicalFinding	pathogenesis of			NULL		0	NULL	NULL	NULL	NULL	NULL	Our study provided evidence that the DISC1 may be the susceptibility gene of autism. It suggested DISC1 might play a role in the pathogenesis of autism.	topic_aut
78550	1	356306	5	NULL	NULL	0	NULL	Clozapine	Chemical		is a type of					second-generation antipsychotic drug	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Clozapine, a second-generation antipsychotic drug known to be effective in the treatment of aggression associated with schizophrenia, has received little attention in ASD.We conducted a retrospective analysis of the changes in disruptive behaviors for all patients with ASD treated with clozapine from 2002 to 2010	topic_aut
78551	3	356306	5	NULL	NULL	NULL	NULL	Clozapine	Chemical		treats		effectively			statement 2	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Clozapine, a second-generation antipsychotic drug known to be effective in the treatment of aggression associated with schizophrenia, has received little attention in ASD.We conducted a retrospective analysis of the changes in disruptive behaviors for all patients with ASD treated with clozapine from 2002 to 2010	topic_aut
78552	2	356306	5	NULL	NULL	0	NULL	aggression	MedicalFinding		is associated with					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Clozapine, a second-generation antipsychotic drug known to be effective in the treatment of aggression associated with schizophrenia, has received little attention in ASD.We conducted a retrospective analysis of the changes in disruptive behaviors for all patients with ASD treated with clozapine from 2002 to 2010	topic_aut
78553	4	356306	5	NULL	NULL	0	NULL	Clozapine	Chemical		is not effective		may			ASD	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	Clozapine, a second-generation antipsychotic drug known to be effective in the treatment of aggression associated with schizophrenia, has received little attention in ASD.We conducted a retrospective analysis of the changes in disruptive behaviors for all patients with ASD treated with clozapine from 2002 to 2010	topic_aut
78554	1	356308	5	NULL	NULL	NULL	NULL	NRXN2	GP	disruption of	is linked to					ASD	MedicalFinding	pathogenesis of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our findings link NRXN2 disruption to the pathogenesis of ASD for the first time and further strengthen the involvement of NRXN1 in SCZ, supporting the notion of a common genetic mechanism in these disorders.	topic_aut
78555	2	356308	5	NULL	NULL	0	NULL	NRXN2	GP		is involved in					SCZ	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings link NRXN2 disruption to the pathogenesis of ASD for the first time and further strengthen the involvement of NRXN1 in SCZ, supporting the notion of a common genetic mechanism in these disorders.	topic_aut
77945	1	356309	7	NULL	NULL	0	NULL	Frequent binge drinking	Chemical		classed as					alcohol misuse	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Frequent binge drinking or getting severely drunk more than twice is classed as alcohol misuse.	topic_bd
78556	1	356310	5	NULL	NULL	0	NULL	autism	MedicalFinding		is associated with					immune dysfunction	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence suggests an association between autism and immune dysfunction. The associations between human lymphocyte antigen (HLA)-A2, B44, DRβ1*04 (DR4), C4B, and haplotype B44-SC30-DR4 and autism have been reported in western countries	topic_aut
78557	2	356310	5	NULL	NULL	0	NULL	(HLA)-A2	GP		is a type of					human lymphocyte antigen	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence suggests an association between autism and immune dysfunction. The associations between human lymphocyte antigen (HLA)-A2, B44, DRβ1*04 (DR4), C4B, and haplotype B44-SC30-DR4 and autism have been reported in western countries	topic_aut
78558	3	356310	5	NULL	NULL	0	NULL	(HLA)-B44	GP		is a type of					human lymphocyte antigen	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence suggests an association between autism and immune dysfunction. The associations between human lymphocyte antigen (HLA)-A2, B44, DRβ1*04 (DR4), C4B, and haplotype B44-SC30-DR4 and autism have been reported in western countries	topic_aut
78559	4	356310	5	NULL	NULL	0	NULL	(HLA)-DR4	GP		is a type of					human lymphocyte antigen	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence suggests an association between autism and immune dysfunction. The associations between human lymphocyte antigen (HLA)-A2, B44, DRβ1*04 (DR4), C4B, and haplotype B44-SC30-DR4 and autism have been reported in western countries	topic_aut
78560	5	356310	5	NULL	NULL	0	NULL	(HLA)-A2	GP		is associated with					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence suggests an association between autism and immune dysfunction. The associations between human lymphocyte antigen (HLA)-A2, B44, DRβ1*04 (DR4), C4B, and haplotype B44-SC30-DR4 and autism have been reported in western countries	topic_aut
78561	6	356310	5	NULL	NULL	0	NULL	(HLA)-B44	GP		is associated with					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence suggests an association between autism and immune dysfunction. The associations between human lymphocyte antigen (HLA)-A2, B44, DRβ1*04 (DR4), C4B, and haplotype B44-SC30-DR4 and autism have been reported in western countries	topic_aut
78562	7	356310	5	NULL	NULL	0	NULL	(HLA)-DR4	GP		is associated with					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence suggests an association between autism and immune dysfunction. The associations between human lymphocyte antigen (HLA)-A2, B44, DRβ1*04 (DR4), C4B, and haplotype B44-SC30-DR4 and autism have been reported in western countries	topic_aut
78563	8	356310	5	NULL	NULL	0	NULL	B44-SC30-DR4	GP		is associated with					autism	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence suggests an association between autism and immune dysfunction. The associations between human lymphocyte antigen (HLA)-A2, B44, DRβ1*04 (DR4), C4B, and haplotype B44-SC30-DR4 and autism have been reported in western countries	topic_aut
78564	1	356311	5	NULL	NULL	0	NULL	L-carnitine	Chemical		improves					mitochondrial dysfunction	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	L-carnitine was proposed as a potential treatment for patients diagnosed with an autism spectrum disorder to improve mitochondrial dysfunction	topic_aut
78565	2	356311	5	NULL	NULL	0	NULL	L-carnitine	Chemical		is a treatment for		potential			autism spectrum disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	L-carnitine was proposed as a potential treatment for patients diagnosed with an autism spectrum disorder to improve mitochondrial dysfunction	topic_aut
78566	1	356312	5	NULL	NULL	NULL	NULL	Desulfovibrio	Organism		is present in					autistic subjects	GroupOfPeople				NULL		NULL	NULL	NULL	NULL	NULL	NULL	However, a recent study of ours employing the powerful pyrosequencing technique on stools of subjects with regressive autism showed that Desulfovibrio was more common in autistic subjects than in controls.	topic_aut
78567	2	356312	5	NULL	NULL	0	NULL	Desulfovibrio	Organism		is present in					controls	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	However, a recent study of ours employing the powerful pyrosequencing technique on stools of subjects with regressive autism showed that Desulfovibrio was more common in autistic subjects than in controls.	topic_aut
78568	3	356312	5	NULL	NULL	0	NULL	statement 1	Process		more common than					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	However, a recent study of ours employing the powerful pyrosequencing technique on stools of subjects with regressive autism showed that Desulfovibrio was more common in autistic subjects than in controls.	topic_aut
78569	1	356313	5	NULL	NULL	0	NULL	ASD	MedicalFinding		is					autism spectrum disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Children with autism spectrum disorders (ASD) are at high risk for oral disease.	topic_aut
78570	2	356313	5	NULL	NULL	0	NULL	ASD children	GroupOfPeople		is at risk of		high			oral disesae	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Children with autism spectrum disorders (ASD) are at high risk for oral disease.	topic_aut
78571	1	356314	5	NULL	NULL	0	NULL	RRBs	MedicalFinding		is					restricted and repetitive behaviors	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Restricted and repetitive behaviors (RRBs) are a core symptom of autism spectrum disorders (ASD).	topic_aut
78572	2	356314	5	NULL	NULL	0	NULL	RRBs	MedicalFinding		is a core symptom of					ASD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Restricted and repetitive behaviors (RRBs) are a core symptom of autism spectrum disorders (ASD).	topic_aut
78573	3	356314	5	NULL	NULL	0	NULL	ASD	MedicalFinding		is					autism spectrum disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Restricted and repetitive behaviors (RRBs) are a core symptom of autism spectrum disorders (ASD).	topic_aut
78574	1	356315	5	NULL	NULL	NULL	NULL	white-matter abnormalities	MedicalFinding		is a key factor in					autism	MedicalFinding	 physiopathology of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Recent evidence points to white-matter abnormalities as a key factor in autism physiopathology	topic_aut
78575	1	356316	5	NULL	NULL	0	NULL	eyeblink synchronization	Process		is absent in					ASD individuals	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	By contrast, the ASD participants did not show any eyeblink synchronization with the speaker, even when viewing the speaker's eyes and mouth simultaneously. The lack of eyeblink entrainment to the speaker in individuals with ASD suggests that they are not able to temporally attune themselves to others' behaviors.	topic_aut
78577	1	356317	5	NULL	NULL	NULL	NULL	High-Functioning Autism individulas	GroupOfPeople		less able to differentiate					language dialects	MentalProcess				NULL		NULL	NULL	NULL	NULL	NULL	NULL	However, the participants with High-Functioning Autism were less able to differentiate among the dialects in a language attitudes task, suggesting that they do not share social stereotypes related to dialect variation with the typically developing comparison group.	topic_aut
77946	1	356318	7	NULL	NULL	0	NULL	Irinotecan	Chemical		activated by					SN-38	Chemical	hydrolysis to			NULL		0	NULL	NULL	NULL	NULL	NULL	Irinotecan is activated by hydrolysis to SN-38, an inhibitor of topoisomerase I.	topic_ccc
77947	2	356318	7	NULL	NULL	0	NULL	SN-38	Chemical		inhibitor of					topoisomerase I	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	Irinotecan is activated by hydrolysis to SN-38, an inhibitor of topoisomerase I.	topic_ccc
77948	1	356320	7	NULL	NULL	NULL	NULL	BAECs	Cell		repress		significantly;;time-dependently			VEGFR2 protein	GP				NULL		NULL	NULL	NULL	NULL	NULL	NULL	In bovine aortic endothelial cells (BAECs), TGF-β1 significantly repressed VEGFR2 protein in a time-dependent and dose-dependent fashion (P < .05).	topic_ccc
77949	2	356320	7	NULL	NULL	0	NULL	BAECs	Cell		repress		significantly;;dose-dependently			VEGFR2 protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	In bovine aortic endothelial cells (BAECs), TGF-β1 significantly repressed VEGFR2 protein in a time-dependent and dose-dependent fashion (P < .05).	topic_ccc
77950	3	356320	7	NULL	NULL	0	NULL	TGF-β1	GP		repress		significantly;;time-dependently			VEGFR2 protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	In bovine aortic endothelial cells (BAECs), TGF-β1 significantly repressed VEGFR2 protein in a time-dependent and dose-dependent fashion (P < .05).	topic_ccc
77951	4	356320	7	NULL	NULL	0	NULL	TGF-β1	GP		repress		significantly;;dose-dependently			VEGFR2 protein	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	In bovine aortic endothelial cells (BAECs), TGF-β1 significantly repressed VEGFR2 protein in a time-dependent and dose-dependent fashion (P < .05).	topic_ccc
77952	5	356320	7	NULL	NULL	0	NULL	BAECs	Cell		is					bovine aortic endothelial cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	In bovine aortic endothelial cells (BAECs), TGF-β1 significantly repressed VEGFR2 protein in a time-dependent and dose-dependent fashion (P < .05).	topic_ccc
77953	1	356323	7	NULL	NULL	0	NULL	bFGF	GP		mitogen for					endothelial cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	 Basic fibroblast growth factor (bFGF) is a mitogen for endothelial cells, which participates in tumor angiogenesis. In vitro, a CTL assay revealed that bFGF-specific cytotoxic T lymphocytes (CTL) resulted in the lysis of mouse microvascular endothelial cells (MS1) rather than that of the CT26 colorectal cancer cells.	topic_ccc
77954	2	356323	7	NULL	NULL	0	NULL	statement 1	Process		participates in					tumor angiogenesis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	 Basic fibroblast growth factor (bFGF) is a mitogen for endothelial cells, which participates in tumor angiogenesis. In vitro, a CTL assay revealed that bFGF-specific cytotoxic T lymphocytes (CTL) resulted in the lysis of mouse microvascular endothelial cells (MS1) rather than that of the CT26 colorectal cancer cells.	topic_ccc
77955	3	356323	7	NULL	NULL	0	NULL	bFGF-specific CTL	Cell		lyse					MS1	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	 Basic fibroblast growth factor (bFGF) is a mitogen for endothelial cells, which participates in tumor angiogenesis. In vitro, a CTL assay revealed that bFGF-specific cytotoxic T lymphocytes (CTL) resulted in the lysis of mouse microvascular endothelial cells (MS1) rather than that of the CT26 colorectal cancer cells.	topic_ccc
77956	4	356323	7	NULL	NULL	0	NULL	bFGF-specific CTL	Cell		does not lyse					CT26 colorectal cancer cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	 Basic fibroblast growth factor (bFGF) is a mitogen for endothelial cells, which participates in tumor angiogenesis. In vitro, a CTL assay revealed that bFGF-specific cytotoxic T lymphocytes (CTL) resulted in the lysis of mouse microvascular endothelial cells (MS1) rather than that of the CT26 colorectal cancer cells.	topic_ccc
77957	5	356323	7	NULL	NULL	0	NULL	bFGF	GP		is					Basic fibroblast growth factor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	 Basic fibroblast growth factor (bFGF) is a mitogen for endothelial cells, which participates in tumor angiogenesis. In vitro, a CTL assay revealed that bFGF-specific cytotoxic T lymphocytes (CTL) resulted in the lysis of mouse microvascular endothelial cells (MS1) rather than that of the CT26 colorectal cancer cells.	topic_ccc
77958	6	356323	7	NULL	NULL	0	NULL	CTL	Cell		is					cytotoxic T lymphocytes 	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	 Basic fibroblast growth factor (bFGF) is a mitogen for endothelial cells, which participates in tumor angiogenesis. In vitro, a CTL assay revealed that bFGF-specific cytotoxic T lymphocytes (CTL) resulted in the lysis of mouse microvascular endothelial cells (MS1) rather than that of the CT26 colorectal cancer cells.	topic_ccc
77959	1	356324	7	NULL	NULL	NULL	NULL	IGF1	GP	SNP rs6214 of	impact on		could			colorectal cancer	MedicalFinding	developing			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our results suggest that the SNP rs6214 of IGF1 could have an impact on developing colorectal cancer and colorectal polyps with villous elements.	topic_ccc
77960	2	356324	7	NULL	NULL	NULL	NULL	IGF1	GP	SNP rs6214 of	impact on		could			colorectal polyps with villous elements	OrganismPart				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our results suggest that the SNP rs6214 of IGF1 could have an impact on developing colorectal cancer and colorectal polyps with villous elements.	topic_ccc
77961	1	356325	7	NULL	NULL	0	NULL	Callosal volume 	OrganismPart	reduction in	observed in					bipolar disorder	MedicalFinding	patients with			NULL		0	NULL	NULL	NULL	NULL	NULL	Callosal volume reduction has been observed in patients with bipolar disorder, but whether these deficits reflect genetic vulnerability to the illness remains unresolved. 	topic_bd
77962	1	356326	7	NULL	NULL	0	NULL	corpus callosum	OrganismPart		is known as					colossal commissure	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	The corpus callosum, also known as the colossal commissure, is a wide, flat bundle of neural fibers beneath the cortex in the eutherian brain at the longitudinal fissure. 	topic_bd
77963	2	356326	7	NULL	NULL	0	NULL	corpus callosum	OrganismPart		is a type of					neural fibers	OrganismPart	wide, flat bundle of 			NULL		0	NULL	NULL	NULL	NULL	NULL	The corpus callosum, also known as the colossal commissure, is a wide, flat bundle of neural fibers beneath the cortex in the eutherian brain at the longitudinal fissure. 	topic_bd
77964	3	356326	7	NULL	NULL	0	NULL	corpus callosum	OrganismPart		located beneath					eutherian brain 	OrganismPart	the cortex in			NULL		0	NULL	NULL	NULL	NULL	NULL	The corpus callosum, also known as the colossal commissure, is a wide, flat bundle of neural fibers beneath the cortex in the eutherian brain at the longitudinal fissure. 	topic_bd
77965	4	356326	7	NULL	NULL	0	NULL	eutherian brain	OrganismPart		occur at					longitudinal fissure	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	The corpus callosum, also known as the colossal commissure, is a wide, flat bundle of neural fibers beneath the cortex in the eutherian brain at the longitudinal fissure. 	topic_bd
77966	1	356327	7	NULL	NULL	NULL	NULL	corpus collosum	OrganismPart	reduction of genu areas of	correlated with		significantly			verbal processing	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	In bipolar probands and co-twins, reduction of genu and splenium midsagittal areas  of the corpus collosum were significantly correlated with verbal processing speed and response inhibition. 	topic_bd
77967	2	356327	7	NULL	NULL	0	NULL	corpus callosum	OrganismPart	reduction of splenium midsagittal areas of	correlated with		significantly			response inhibition	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	In bipolar probands and co-twins, reduction of genu and splenium midsagittal areas  of the corpus collosum were significantly correlated with verbal processing speed and response inhibition. 	topic_bd
77968	3	356327	7	NULL	NULL	0	NULL	statement 1	Process		occur in					bipolar probands	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In bipolar probands and co-twins, reduction of genu and splenium midsagittal areas  of the corpus collosum were significantly correlated with verbal processing speed and response inhibition. 	topic_bd
77969	4	356327	7	NULL	NULL	0	NULL	statement 1	Process		occur in					co-twins	Person				NULL		0	NULL	NULL	NULL	NULL	NULL	In bipolar probands and co-twins, reduction of genu and splenium midsagittal areas  of the corpus collosum were significantly correlated with verbal processing speed and response inhibition. 	topic_bd
77970	5	356327	7	NULL	NULL	0	NULL	statement 2	Process		occur in					bipolar probands	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In bipolar probands and co-twins, reduction of genu and splenium midsagittal areas  of the corpus collosum were significantly correlated with verbal processing speed and response inhibition. 	topic_bd
77971	6	356327	7	NULL	NULL	0	NULL	statement 2	Process		occur in					co-twins	Person				NULL		0	NULL	NULL	NULL	NULL	NULL	In bipolar probands and co-twins, reduction of genu and splenium midsagittal areas  of the corpus collosum were significantly correlated with verbal processing speed and response inhibition. 	topic_bd
77972	1	356328	7	NULL	NULL	0	NULL	callosal thinning	OrganismPart		appear to be					disease 	MedicalFinding	related to			NULL		0	NULL	NULL	NULL	NULL	NULL	However, findings of callosal thinning appear to be disease related, rather than reflecting genetic vulnerability to bipolar illness. 	topic_bd
77973	2	356328	7	NULL	NULL	NULL	NULL	callosal thinning	Process		does not reflect					bipolar illness	MedicalFinding	genetic vulnerability to			NULL		NULL	NULL	NULL	NULL	NULL	NULL	However, findings of callosal thinning appear to be disease related, rather than reflecting genetic vulnerability to bipolar illness. 	topic_bd
77974	1	356329	7	NULL	NULL	0	NULL	pineal gland	OrganismPart	putative dysfunction of 	not related to		directly			pineal gland	OrganismPart	abnormal volume of			NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the putative dysfunction of the pineal gland in bipolar disorder could be not directly related to an abnormal volume of the pineal gland.	topic_bd
77975	2	356329	7	NULL	NULL	0	NULL	statement 1	Process		occur in					bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the putative dysfunction of the pineal gland in bipolar disorder could be not directly related to an abnormal volume of the pineal gland.	topic_bd
77976	1	356330	7	NULL	NULL	0	NULL	SNP (rs13438494)	NucleicAcid		intron of					PCLO gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	One SNP (rs13438494), in an intron of the piccolo (PCLO) gene, was significantly associated with bipolar disorder  in the meta-analysis of GWAS.	topic_bd
77977	2	356330	7	NULL	NULL	0	NULL	SNP (rs13438494)	NucleicAcid		associated with		significantly			bipolar disorder	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	One SNP (rs13438494), in an intron of the piccolo (PCLO) gene, was significantly associated with bipolar disorder  in the meta-analysis of GWAS.	topic_bd
77978	3	356330	7	NULL	NULL	0	NULL	PCLO gene	GP		is					piccolo gene	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	One SNP (rs13438494), in an intron of the piccolo (PCLO) gene, was significantly associated with bipolar disorder  in the meta-analysis of GWAS.	topic_bd
77979	1	356331	7	NULL	NULL	0	NULL	SNP	NucleicAcid		is a type of					DNA sequence	NucleicAcid	variation in			NULL		0	NULL	NULL	NULL	NULL	NULL	A single-nucleotide polymorphism (SNP, pronounced snip) is a DNA sequence variation occurring when a single nucleotide in the genome (or other shared sequence) differs between members of a biological species or paired chromosomes in an individual.	topic_bd
77980	2	356331	7	NULL	NULL	0	NULL	statement 1	Process		occur upon 					genome	GP	variation of single nucleotide			NULL		0	NULL	NULL	NULL	NULL	NULL	A single-nucleotide polymorphism (SNP, pronounced snip) is a DNA sequence variation occurring when a single nucleotide in the genome (or other shared sequence) differs between members of a biological species or paired chromosomes in an individual.	topic_bd
77981	3	356331	7	NULL	NULL	0	NULL	statement 2	Process		occur between					biological species	Organism	members of			NULL		0	NULL	NULL	NULL	NULL	NULL	A single-nucleotide polymorphism (SNP, pronounced snip) is a DNA sequence variation occurring when a single nucleotide in the genome (or other shared sequence) differs between members of a biological species or paired chromosomes in an individual.	topic_bd
77982	4	356331	7	NULL	NULL	0	NULL	statement 2	Process		occur between					individual	Person	paired chromosomes in			NULL		0	NULL	NULL	NULL	NULL	NULL	A single-nucleotide polymorphism (SNP, pronounced snip) is a DNA sequence variation occurring when a single nucleotide in the genome (or other shared sequence) differs between members of a biological species or paired chromosomes in an individual.	topic_bd
77983	5	356331	7	NULL	NULL	0	NULL	statement 3	Process		is an alternative to					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	A single-nucleotide polymorphism (SNP, pronounced snip) is a DNA sequence variation occurring when a single nucleotide in the genome (or other shared sequence) differs between members of a biological species or paired chromosomes in an individual.	topic_bd
77984	6	356331	7	NULL	NULL	0	NULL	SNP	Process		is					single-nucleotide polymorphism	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	A single-nucleotide polymorphism (SNP, pronounced snip) is a DNA sequence variation occurring when a single nucleotide in the genome (or other shared sequence) differs between members of a biological species or paired chromosomes in an individual.	topic_bd
78578	1	356333	5	NULL	NULL	NULL	NULL	DUI	MedicalFinding		is not correlated to		significantly			brain	OrganismPart	change in volume of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	We found no significant correlation between DUI and brain volume (change) in schizophrenia patients.	topic_sch
78579	2	356333	5	NULL	NULL	NULL	NULL	statement 1	Process		occurs in					schizophrenia patients	GroupOfPeople				NULL		NULL	NULL	NULL	NULL	NULL	NULL	We found no significant correlation between DUI and brain volume (change) in schizophrenia patients.	topic_sch
78580	1	356334	5	NULL	NULL	0	NULL	Schizophrenic patients	GroupOfPeople		identify					emotions	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	In the first experiment, we found that patients with schizophrenia were less accurate at identifying emotions than a group of matched controls.	topic_sch
78581	2	356334	5	NULL	NULL	0	NULL	controls	GroupOfPeople		identify					emotions	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	In the first experiment, we found that patients with schizophrenia were less accurate at identifying emotions than a group of matched controls.	topic_sch
78582	3	356334	5	NULL	NULL	0	NULL	statement 1	Process		less accurate than					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	In the first experiment, we found that patients with schizophrenia were less accurate at identifying emotions than a group of matched controls.	topic_sch
78583	1	356335	5	NULL	NULL	0	NULL	oxytocin	GP	administration of	improves					schizophrenia	MedicalFinding	clinical symptoms of			NULL		0	NULL	NULL	NULL	NULL	NULL	nterest in oxytocin in schizophrenia is just beginning to emerge. Recent studies have shown improvements in clinical symptoms, including both positive and negative symptoms, with oxytocin administration (Feifel et al. 2010; Rubin et al. 2010). 	topic_sch
78584	1	356337	5	NULL	NULL	0	NULL	oxytocin	GP		effects		beneficial			emotion recognition	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Complementing this, our results suggest that oxytocin can have beneficial effects on emotion recognition, a well-documented deficit in this clinical population, which may have an impact on symptoms in the longer term, as differences were only evident after 3 weeks of treatment (Feifel et al. 2010), as well as contributing to better social functioning in the patients. Our study also demonstrates acute improvements in emotion recognition. This offers the potential in the future of integrating oxytocin treatment with psychological therapy using the window of opportunity created by the acute oxytocin effects.	topic_sch
78585	2	356337	5	NULL	NULL	0	NULL	statement 1	Process		contribute to					social functioning	Process	better			NULL		0	NULL	NULL	NULL	NULL	NULL	Complementing this, our results suggest that oxytocin can have beneficial effects on emotion recognition, a well-documented deficit in this clinical population, which may have an impact on symptoms in the longer term, as differences were only evident after 3 weeks of treatment (Feifel et al. 2010), as well as contributing to better social functioning in the patients. Our study also demonstrates acute improvements in emotion recognition. This offers the potential in the future of integrating oxytocin treatment with psychological therapy using the window of opportunity created by the acute oxytocin effects.	topic_sch
78586	1	356338	5	NULL	NULL	0	NULL	rs3016384	NucleicAcid		is a type of					SNP	NucleicAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	The previously discovered SNP associated with schizophrenia in Europeans, rs3016384, also showed significant association with schizophrenia in the Thai population [P = 0.01; odds ratio of the minor T allele, 0.59 (0.44-0.79)]. Therefore, the OPCML gene is considered to be a schizophrenia-susceptible gene in the Thai population.	topic_sch
78587	2	356338	5	NULL	NULL	0	NULL	rs3016384	NucleicAcid		is associated with					schizophrenia	MedicalFinding				NULL	Europeans	0	NULL	NULL	NULL	NULL	NULL	The previously discovered SNP associated with schizophrenia in Europeans, rs3016384, also showed significant association with schizophrenia in the Thai population [P = 0.01; odds ratio of the minor T allele, 0.59 (0.44-0.79)]. Therefore, the OPCML gene is considered to be a schizophrenia-susceptible gene in the Thai population.	topic_sch
78588	3	356338	5	NULL	NULL	0	NULL	statement 2	Process		is associated with					schizophrenia	MedicalFinding				NULL	Thai population	0	NULL	NULL	NULL	NULL	NULL	The previously discovered SNP associated with schizophrenia in Europeans, rs3016384, also showed significant association with schizophrenia in the Thai population [P = 0.01; odds ratio of the minor T allele, 0.59 (0.44-0.79)]. Therefore, the OPCML gene is considered to be a schizophrenia-susceptible gene in the Thai population.	topic_sch
78589	4	356338	5	NULL	NULL	0	NULL	OPCML gene	GP		 is considered to be					schizophrenia-susceptible gene	GP				NULL	Thai population	0	NULL	NULL	NULL	NULL	NULL	The previously discovered SNP associated with schizophrenia in Europeans, rs3016384, also showed significant association with schizophrenia in the Thai population [P = 0.01; odds ratio of the minor T allele, 0.59 (0.44-0.79)]. Therefore, the OPCML gene is considered to be a schizophrenia-susceptible gene in the Thai population.	topic_sch
78590	1	356339	5	NULL	NULL	0	NULL	cortical-striatal disconnection	Process		occurs within					CON	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that schizophrenia is associated with cortical-striatal disconnection within the CON. The result provides a network basis for the cortico-striatal disconnection hypothesis of schizophrenia.	topic_sch
78591	2	356339	5	NULL	NULL	0	NULL	schizophrenia	MedicalFinding		is associated with					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that schizophrenia is associated with cortical-striatal disconnection within the CON. The result provides a network basis for the cortico-striatal disconnection hypothesis of schizophrenia.	topic_sch
78592	1	356340	5	NULL	NULL	0	NULL	gamma oscillations	PhysicalPhenomenon	abnormal	reported in					SCZ patients	GroupOfPeople				NULL		0	NULL	NULL	NULL	NULL	NULL	For patients with schizophrenia (SCZ), a disease associated with poor cognition, abnormal gamma oscillations have been reported in many experimental paradigms. 	topic_sch
78593	2	356340	5	NULL	NULL	0	NULL	SCZ	MedicalFinding		is associated with					poor cognition	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	For patients with schizophrenia (SCZ), a disease associated with poor cognition, abnormal gamma oscillations have been reported in many experimental paradigms. 	topic_sch
78594	3	356340	5	NULL	NULL	0	NULL	SCZ	MedicalFinding		is					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	For patients with schizophrenia (SCZ), a disease associated with poor cognition, abnormal gamma oscillations have been reported in many experimental paradigms. 	topic_sch
78595	1	356341	5	NULL	NULL	0	NULL	γ oscillations	PhysicalPhenomenon	irregular	serve as		may			schizophrenia	MedicalFinding	endophenotypes of			NULL		0	NULL	NULL	NULL	NULL	NULL	Irregular γ oscillations may serve as endophenotypes for schizophrenia. 	topic_sch
78596	1	356342	5	NULL	NULL	0	NULL	schizophrenia	MedicalFinding		is associated with					DLPFC	GP	neurobiological abnormalities of			NULL		0	NULL	NULL	NULL	NULL	NULL	Schizophrenia is associated with neurobiological abnormalities in the DLPFC. 	topic_sch
78597	1	356344	5	NULL	NULL	0	NULL	oxytocin	GP	intranasal	reduce					schizophrenia	MedicalFinding	psychotic symptoms of			NULL		0	NULL	NULL	NULL	NULL	NULL	Intranasal oxytocin reduces psychotic symptoms and improves Theory of Mind and social perception in schizophrenia.	topic_sch
78598	2	356344	5	NULL	NULL	0	NULL	oxytocin	GP	intranasal	improves					schizophrenic	GroupOfPeople	social perception of			NULL		0	NULL	NULL	NULL	NULL	NULL	Intranasal oxytocin reduces psychotic symptoms and improves Theory of Mind and social perception in schizophrenia.	topic_sch
78599	3	356344	5	NULL	NULL	0	NULL	oxytocin	GP	intranasal	improves					schizophrenic	GroupOfPeople	Theory of Mind of			NULL		0	NULL	NULL	NULL	NULL	NULL	Intranasal oxytocin reduces psychotic symptoms and improves Theory of Mind and social perception in schizophrenia.	topic_sch
77985	1	356345	7	NULL	NULL	0	NULL	APL	MedicalFinding		subtype of					AML	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Acute promyelocytic leukemia (APL) is a subtype of the cancer acute myeloid leukemia (AML).	topic_ll
77986	2	356345	7	NULL	NULL	0	NULL	APL	MedicalFinding		is					Acute promyelocytic leukemia 	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Acute promyelocytic leukemia (APL) is a subtype of the cancer acute myeloid leukemia (AML).	topic_ll
77987	3	356345	7	NULL	NULL	0	NULL	AML	MedicalFinding		is					acute myeloid leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Acute promyelocytic leukemia (APL) is a subtype of the cancer acute myeloid leukemia (AML).	topic_ll
77988	4	356345	7	NULL	NULL	0	NULL	APL	MedicalFinding		subtype of					cancer	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Acute promyelocytic leukemia (APL) is a subtype of the cancer acute myeloid leukemia (AML).	topic_ll
77989	1	356346	7	NULL	NULL	NULL	NULL	Tumor vascularization	Process		occur in					lymphoma tissues	OrganismPart				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Tumor vascularization is higher in lymphoma tissue than in reactive lymph nodes and increases in step with clinically more aggressive lymphoma subtypes and advanced-stage disease.	topic_ll
77990	2	356346	7	NULL	NULL	0	NULL	Tumor vascularization	Process		occur in					reactive lymph nodes	OrganismPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor vascularization is higher in lymphoma tissue than in reactive lymph nodes and increases in step with clinically more aggressive lymphoma subtypes and advanced-stage disease.	topic_ll
77991	3	356346	7	NULL	NULL	0	NULL	statement 1	Process		is higher than					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor vascularization is higher in lymphoma tissue than in reactive lymph nodes and increases in step with clinically more aggressive lymphoma subtypes and advanced-stage disease.	topic_ll
77992	4	356346	7	NULL	NULL	0	NULL	Tumor vascularization	Process		increases					lymphoma subtypes	MedicalFinding	in step with more aggressive			NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor vascularization is higher in lymphoma tissue than in reactive lymph nodes and increases in step with clinically more aggressive lymphoma subtypes and advanced-stage disease.	topic_ll
77993	1	356347	7	NULL	NULL	0	NULL	gene transfer therapy 	MedicalProcedure		create					"serial killer" T cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	The findings, published simultaneously in the New England Journal of Medicine and Science Translational Medicine on August 10, are the first demonstration of the use of gene transfer therapy to create "serial killer" T cells aimed at cancerous tumors.	topic_ll
77994	2	356347	7	NULL	NULL	0	NULL	"serial killer" T cells	Cell		aimed at					cancerous tumors	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The findings, published simultaneously in the New England Journal of Medicine and Science Translational Medicine on August 10, are the first demonstration of the use of gene transfer therapy to create "serial killer" T cells aimed at cancerous tumors.	topic_ll
77995	1	356348	7	NULL	NULL	0	NULL	CLL	MedicalFinding		treated with					T cells	Cell	genetically engineered versions of their own			NULL		0	NULL	NULL	NULL	NULL	NULL	In a cancer treatment breakthrough 20 years in the making, researchers from the University of Pennsylvania's Abramson Cancer Center and Perelman School of Medicine have shown sustained remissions of up to a year among a small group of advanced chronic lymphocytic leukemia (CLL) patients treated with genetically engineered versions of their own T cells.	topic_ll
77996	2	356348	7	NULL	NULL	0	NULL	CLL	MedicalFinding		is					chronic lymphocytic leukemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	In a cancer treatment breakthrough 20 years in the making, researchers from the University of Pennsylvania's Abramson Cancer Center and Perelman School of Medicine have shown sustained remissions of up to a year among a small group of advanced chronic lymphocytic leukemia (CLL) patients treated with genetically engineered versions of their own T cells.	topic_ll
77997	1	356349	7	NULL	NULL	0	NULL	NOC intake	Chemical	human	associated with					leukemia	MedicalFinding	risk of			NULL		0	NULL	NULL	NULL	NULL	NULL	While these results are compatible with the experimental animal literature and the hypothesis that human NOC intake is associated with leukemia risk, given potential biases in the data, further study of this hypothesis with more focused and comprehensive epidemiologic studies is warranted.	topic_ll
77998	1	356351	7	NULL	NULL	0	NULL	ISCs	Cell	gene signature specific for adult	predicts					disease relapse	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Here, we report that a gene signature specific for adult intestinal stem cells (ISCs) predicts disease relapse in CRC patients.	topic_ccc
77999	2	356351	7	NULL	NULL	0	NULL	statement 1	Process		occur in					CRC	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Here, we report that a gene signature specific for adult intestinal stem cells (ISCs) predicts disease relapse in CRC patients.	topic_ccc
78000	3	356351	7	NULL	NULL	0	NULL	ISCs	Cell		is					intestinal stem cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Here, we report that a gene signature specific for adult intestinal stem cells (ISCs) predicts disease relapse in CRC patients.	topic_ccc
78600	1	356352	5	NULL	NULL	0	NULL	D-serine	AminoAcid		is a coagonist of					NMDA receptor	GP				NULL		0	NULL	NULL	NULL	NULL	NULL	The NMDA receptor coagonist D-serine is important in a number of different processes in the central nervous system, ranging from synaptic plasticity to disease states, including schizophrenia.	topic_sch
78601	2	356352	5	NULL	NULL	0	NULL	D-serine	AminoAcid		is important in					central nervous system	OrganismPart	different processes of			NULL		0	NULL	NULL	NULL	NULL	NULL	The NMDA receptor coagonist D-serine is important in a number of different processes in the central nervous system, ranging from synaptic plasticity to disease states, including schizophrenia.	topic_sch
78602	3	356352	5	NULL	NULL	0	NULL	central nervous system	OrganismPart	different processes of	range from					synaptic plasticity	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The NMDA receptor coagonist D-serine is important in a number of different processes in the central nervous system, ranging from synaptic plasticity to disease states, including schizophrenia.	topic_sch
78603	4	356352	5	NULL	NULL	0	NULL	central nervous system	OrganismPart	different processes of	range to					disease states	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The NMDA receptor coagonist D-serine is important in a number of different processes in the central nervous system, ranging from synaptic plasticity to disease states, including schizophrenia.	topic_sch
78604	5	356352	5	NULL	NULL	0	NULL	statement 3	Process		occurs along with					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The NMDA receptor coagonist D-serine is important in a number of different processes in the central nervous system, ranging from synaptic plasticity to disease states, including schizophrenia.	topic_sch
78605	6	356352	5	NULL	NULL	0	NULL	disease states	MedicalFinding		include					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The NMDA receptor coagonist D-serine is important in a number of different processes in the central nervous system, ranging from synaptic plasticity to disease states, including schizophrenia.	topic_sch
78606	1	356354	5	NULL	NULL	0	NULL	type-1 immune response	Process	capacity of	reduced in					schizophrenia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The decreased response of lymphocytes after stimulation with specific antigens reflects a reduced capacity for a type-1 immune response in schizophrenia, as well (Müller et al., 1991).	topic_sch
79630	1	356557	5	NULL	NULL	0	NULL	Bazedoxifene	NonProteinOrNucleicAcidChemical		is a type of					SERM	NonProteinOrNucleicAcidChemical	new-generation			NULL		0	NULL	NULL	NULL	NULL	NULL	( Bazedoxifene as a new-generation SERM ) .	manualset1
79631	1	356563	5	NULL	NULL	0	NULL	Biatrial re-synchronization	MedicalProcedure		is used to treat					Biatrial re-synchronization	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Biatrial re-synchronization in the treatment of paroxysmal atrial fibrillation .	manualset1
79632	1	356590	5	NULL	NULL	0	NULL	dead fetus	BodyPart	retension of	causes					coagulation disorder	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( COAGULATION DISORDERS CAUSED BY RETENTION OF A DEAD FETUS AND THEIR MANAGEMENT ) .	manualset1
79638	1	356592	5	NULL	NULL	0	NULL	Haurydrin	NonProteinOrNucleicAcidChemical		effects		may			Diuresis	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( CONTRIBUTION ON THE EFFECT OF HAURYDRIN ON DIURESIS AND ON THE ELECTROLYTE BALANCE ) .	manualset1
79639	2	356592	5	NULL	NULL	NULL	NULL	Haurydrin	NonProteinOrNucleicAcidChemical		effects		may			Electrolyte balance	BiologicalProcess				NULL		NULL	NULL	NULL	NULL	NULL	NULL	( CONTRIBUTION ON THE EFFECT OF HAURYDRIN ON DIURESIS AND ON THE ELECTROLYTE BALANCE ) .	manualset1
79640	1	356605	5	NULL	NULL	0	NULL	Capillary sprouting	Process		is a type of					reparation	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	( Capillary sprouting as a reparation principle in local radiation injuries ) .	manualset1
79641	2	356605	5	NULL	NULL	0	NULL	statement 1	Process		occurs in					radiation injuries	MedicalFinding	local			NULL		0	NULL	NULL	NULL	NULL	NULL	( Capillary sprouting as a reparation principle in local radiation injuries ) .	manualset1
79642	1	356607	5	NULL	NULL	0	NULL	pneumatic dilatation	MedicalFinding		occurs in					achalasia	Disease				NULL	esophagus	0	NULL	NULL	NULL	NULL	NULL	( Cardiac arrhythmia during pneumatic dilatation of achalasia of the esophagus ( author 's transl ) ) .	manualset1
79643	2	356607	5	NULL	NULL	0	NULL	statement 1	Process		leads to					Cardiac arrhythmia	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Cardiac arrhythmia during pneumatic dilatation of achalasia of the esophagus ( author 's transl ) ) .	manualset1
79644	1	356608	5	NULL	NULL	0	NULL	cigarette smoking	Process		leads to					Cardiac responses	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Cardiac responses to cigarette smoking in healthy young male adults ( author 's transl ) ) .	manualset1
79645	2	356608	5	NULL	NULL	0	NULL	statement 1	Process		occurs in					male adults	PersonGroup	healthy;;young			NULL		0	NULL	NULL	NULL	NULL	NULL	( Cardiac responses to cigarette smoking in healthy young male adults ( author 's transl ) ) .	manualset1
79646	1	356616	5	NULL	NULL	0	NULL	neuromyelitis optica	Disease		suspected to be					toxoplasmosis	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Case of neuromyelitis optica suspected to be toxoplasmosis ) .	manualset1
79647	1	356618	5	NULL	NULL	0	NULL	septicemia	Disease		is caused by					Clostridium perfringens	Organism	infection of;;postabortal			NULL		0	NULL	NULL	NULL	NULL	NULL	( Case of septicemia caused by postabortal Clostridium perfringens infection with anuria treated by exchange transfusion and tifomycin ) .	manualset1
79648	1	356621	5	NULL	NULL	0	NULL	all-trans retinoic acid	NonProteinOrNucleicAcidChemical		is used to treat					leukemia	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Central nervous system relapse with multiple brain masses in an acute promyelocytic leukemia patient treated with all-trans retinoic acid ) .	manualset1
79649	1	356626	5	NULL	NULL	0	NULL	Cerebral aneurysm	Disease		is associated with					persistent trigeminal artery	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	( Cerebral aneurysm associated with persistent trigeminal artery and occlusion of the subclavian artery .	manualset1
79650	2	356626	5	NULL	NULL	0	NULL	Cerebral aneurysm	Disease		is associated with					subclavian artery	BodyPart	occlusion of			NULL		0	NULL	NULL	NULL	NULL	NULL	( Cerebral aneurysm associated with persistent trigeminal artery and occlusion of the subclavian artery .	manualset1
79651	1	356628	5	NULL	NULL	0	NULL	intracranial tumors	Disease	unsuspected	leads to					Cerebral hemorrhage	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Cerebral hemorrhage from unsuspected intracranial tumors ) .	manualset1
79652	1	356631	5	NULL	NULL	0	NULL	Cervical lymph node	BodyPart		metastases from					primary tumor	Disease	unknown			NULL		0	NULL	NULL	NULL	NULL	NULL	( Cervical lymph node metastases from an unknown primary tumor ) .	manualset1
79653	1	356636	5	NULL	NULL	0	NULL	erthrocytes	Cell	acidic resistance of	changes in		may			psychiatric disorders	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Changes in the acidic resistance of erythrocytes in psychiatric disorders ( author 's transl ) ) .	manualset1
79654	1	356637	5	NULL	NULL	0	NULL	chromatin	Chromosome	compactness of;;nucleosome	changes during					aging	BiologicalProcess				NULL	bovine liver	0	NULL	NULL	NULL	NULL	NULL	( Changes in the compactness of nucleosome chromatin from the bovine liver during aging ) .	manualset1
79655	1	356643	5	NULL	NULL	0	NULL	TNF-alpha	Protein		changes in					silicosis patients	PersonGroup				NULL		0	NULL	NULL	NULL	NULL	NULL	( Changes of TNF-alpha and C ( 3 ) complements in patients with silicosis ) .	manualset1
79656	2	356643	5	NULL	NULL	0	NULL	C ( 3 ) complements	Protein		changes in					silicosis patients	PersonGroup				NULL		0	NULL	NULL	NULL	NULL	NULL	( Changes of TNF-alpha and C ( 3 ) complements in patients with silicosis ) .	manualset1
79657	1	356654	5	NULL	NULL	0	NULL	Chlormezanone	NonProteinOrNucleicAcidChemical		is a type of					Chlormezanone	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	( Chlormezanone : muscle relaxant and neuropsychic normalizer .	manualset1
79658	2	356654	5	NULL	NULL	0	NULL	Chlormezanone	NonProteinOrNucleicAcidChemical		is a type of					neuropsychic normalizer	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	( Chlormezanone : muscle relaxant and neuropsychic normalizer .	manualset1
79659	1	356661	5	NULL	NULL	0	NULL	Toxocara canis	Organism		causes					Chronic endophthalmitis	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Chronic endophthalmitis due to Toxocara canis ) .	manualset1
79660	1	356685	5	NULL	NULL	0	NULL	radiation synovectomy	MedicalProcedure		treats					chronic synovitis					NULL	knee joint	0	NULL	NULL	NULL	NULL	NULL	( Clinical experience with radiation synovectomy in the treatment of chronic synovitis of the knee joint -- long-term investigation ( author 's transl ) ) .	manualset1
79670	1	356764	5	NULL	NULL	0	NULL	ventricular tachycardia	Disease		is controlled by					ventricle	BodyPart	rapid electric stimulation of			NULL		0	NULL	NULL	NULL	NULL	NULL	( Control of ventricular tachycardia by rapid electric stimulation of the ventricle ) .	manualset1
79671	1	356765	5	NULL	NULL	0	NULL	Conus venoms	Protein		is a source of					toxins	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	( Conus venoms : a source of toxins which interact with membrane - potential-dependent sodium channels ) .	manualset1
79672	2	356765	5	NULL	NULL	0	NULL	Conus venoms	Protein		interacts with					membrane - potential-dependent sodium channels	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	( Conus venoms : a source of toxins which interact with membrane - potential-dependent sodium channels ) .	manualset1
79673	1	356790	5	NULL	NULL	0	NULL	Cutaneous giant cell tubercle	Disease		is induced by					tuberculin	Organism	desensitization with			NULL		0	NULL	NULL	NULL	NULL	NULL	( Cutaneous giant cell tubercle induced by desensitization with old tuberculin ( Koch ) ) .	manualset1
79674	1	356794	5	NULL	NULL	0	NULL	Cystic pulmonary metastasis	Disease		stimulates					histiocytosis X	Disease	diagnosis of			NULL		0	NULL	NULL	NULL	NULL	NULL	( Cystic pulmonary metastasis simulating a diagnosis of histiocytosis X ) .	manualset1
79675	1	356805	5	NULL	NULL	NULL	NULL	macular ganglion cell complex	AnatomicalPart		is damaged in					multiple sclerosis	Disease				NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Damage of macular ganglion cell complex and peripapillary retinal nerve fiber layer in multiple sclerosis ) .	manualset1
79676	2	356805	5	NULL	NULL	0	NULL	peripapillary retinal nerve fiber layer	AnatomicalPart		is damaged in					multiple sclerosis	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Damage of macular ganglion cell complex and peripapillary retinal nerve fiber layer in multiple sclerosis ) .	manualset1
79677	1	356809	5	NULL	NULL	0	NULL	Vim nucleus	BodyPart	stimulation of	plays a role in					parkinsonian tremor	Disease	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	( Deep brain stimulation of the Vim nucleus of the thalamus in the treatment of parkinsonian tremor ) .	manualset1
79678	2	356809	5	NULL	NULL	0	NULL	Vim nucleus	BodyPart		is present in					thalamus	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	( Deep brain stimulation of the Vim nucleus of the thalamus in the treatment of parkinsonian tremor ) .	manualset1
79679	3	356809	5	NULL	NULL	0	NULL	statement 2	BodyPart		is a part of					deep brain	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	( Deep brain stimulation of the Vim nucleus of the thalamus in the treatment of parkinsonian tremor ) .	manualset1
80647	1	356855	5	NULL	NULL	0	NULL	imatinib mesylate	NonProteinOrNucleicAcidChemical		treats					Philadelphia chromosome-positive chronic myelogenous leukemia patients	PersonGroup				NULL		0	NULL	NULL	NULL	NULL	NULL	( Disease transformation in imatinib mesylate treated Philadelphia chromosome-positive chronic myelogenous leukemia patients achieved cytogenetic remissions ) .	manualset1
80648	2	356855	5	NULL	NULL	0	NULL	statement 1	Process	disease transformation of	achieved					cytogenetic remissions	BiologicalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	( Disease transformation in imatinib mesylate treated Philadelphia chromosome-positive chronic myelogenous leukemia patients achieved cytogenetic remissions ) .	manualset1
79680	1	356890	5	NULL	NULL	0	NULL	1,3 butylene glycol	NonProteinOrNucleicAcidChemical		effects		may			reproduction	BiologicalProcess				NULL	rat	0	NULL	NULL	NULL	NULL	NULL	( Effect of 1,3 butylene glycol on reproduction in rats ) .	manualset1
79681	1	356891	5	NULL	NULL	0	NULL	ACTH	GeneOrProtein		effects		may			mortality	BiologicalProcess				NULL	irradiated mice	0	NULL	NULL	NULL	NULL	NULL	( Effect of ACTH on mortality of irradiated mice ) .	manualset1
79682	1	356892	5	NULL	NULL	0	NULL	BAL	Chemical		effects		may			pencillin	NonProteinOrNucleicAcidChemical	inhibitory property of			NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of BAL on the inhibitory property of penicillin and streptomycin ) .	manualset1
79683	2	356892	5	NULL	NULL	0	NULL	BAL	Chemical		effects		may			streptomycin	NonProteinOrNucleicAcidChemical	inhibitory property of			NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of BAL on the inhibitory property of penicillin and streptomycin ) .	manualset1
79684	1	356897	5	NULL	NULL	0	NULL	dexamethasone	NonProteinOrNucleicAcidChemical		effects		may			phospholipid spectrum	NonProteinOrNucleicAcidChemical	skin			NULL	laboratory animals	0	NULL	NULL	NULL	NULL	NULL	( Effect of dexamethasone on skin phospholipid spectrum in laboratory animals ) .	manualset1
79685	1	356898	5	NULL	NULL	0	NULL	olive oil	NonProteinOrNucleicAcidChemical	dietary	effects		may			high density lipoproteins	NonProteinOrNucleicAcidChemical	plasma			NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of dietary olive oil on plasma high density lipoproteins ) .	manualset1
79686	1	356899	5	NULL	NULL	0	NULL	diet	Food		contains					caloric levels	Measurement	different			NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of diets with different caloric levels on blood protein turnover ) .	manualset1
79687	2	356899	5	NULL	NULL	0	NULL	statement 1	Process		effects		may			protein	Protein	turnover of;;blood			NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of diets with different caloric levels on blood protein turnover ) .	manualset1
79693	1	356901	5	NULL	NULL	0	NULL	erythromycin	NonProteinOrNucleicAcidChemical		effects		may			polymorphonuclear leukocyte	Cell	ingestion of;;human			NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of erythromycin and phosphomycin on the ingestion and destruction capacity of the human polymorphonuclear leukocyte ) .	manualset1
79694	3	356901	5	NULL	NULL	0	NULL	erythromycin	NonProteinOrNucleicAcidChemical		effects		may			statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of erythromycin and phosphomycin on the ingestion and destruction capacity of the human polymorphonuclear leukocyte ) .	manualset1
79695	2	356901	5	NULL	NULL	0	NULL	polymorphonuclear leukocyte	Cell	human	is involved in					destruction	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of erythromycin and phosphomycin on the ingestion and destruction capacity of the human polymorphonuclear leukocyte ) .	manualset1
79696	4	356901	5	NULL	NULL	0	NULL	phosphomycin	NonProteinOrNucleicAcidChemical		effects		may			polymorphonuclear leukocyte	Cell	ingestion of;;human			NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of erythromycin and phosphomycin on the ingestion and destruction capacity of the human polymorphonuclear leukocyte ) .	manualset1
79697	5	356901	5	NULL	NULL	0	NULL	phosphomycin	NonProteinOrNucleicAcidChemical		effects		may			statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of erythromycin and phosphomycin on the ingestion and destruction capacity of the human polymorphonuclear leukocyte ) .	manualset1
79698	1	356902	5	NULL	NULL	NULL	NULL	gestrinone	NonProteinOrNucleicAcidChemical		effects		may			lipid	NonProteinOrNucleicAcidChemical	metabolic parameters of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Effect of gestrinone on the lipid metabolic parameters and bone mineral density in patients with endometriosis ) .	manualset1
79699	2	356902	5	NULL	NULL	0	NULL	statement 1	Process		occurs in					endometriosis patients	PersonGroup				NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of gestrinone on the lipid metabolic parameters and bone mineral density in patients with endometriosis ) .	manualset1
79700	3	356902	5	NULL	NULL	0	NULL	gestrinone	NonProteinOrNucleicAcidChemical		effects		may			bone	BodyPart	mineral density of			NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of gestrinone on the lipid metabolic parameters and bone mineral density in patients with endometriosis ) .	manualset1
79701	4	356902	5	NULL	NULL	0	NULL	statement 3	Process		occurs in					endometriosis patients	PersonGroup				NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of gestrinone on the lipid metabolic parameters and bone mineral density in patients with endometriosis ) .	manualset1
79702	1	356903	5	NULL	NULL	0	NULL	glycosylation	MolecularProcess		effects		may			collagen type I fibrillogenesis	MolecularProcess				NULL	connective tissue	0	NULL	NULL	NULL	NULL	NULL	( Effect of glycosylation on collagen type I fibrillogenesis in a model of connective tissue ) .	manualset1
79703	1	356905	5	NULL	NULL	0	NULL	phenol	NonProteinOrNucleicAcidChemical		effects		may			V79 cells	Cell	cultured			NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of phenol on cultured V79 cells ) .	manualset1
79704	1	356906	5	NULL	NULL	0	NULL	physical exercise	Process		effects		may			bone tissue	BodyPart	calcified			NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of physical exercise on calcified bone tissue ) .	manualset1
79705	1	356907	5	NULL	NULL	NULL	NULL	lactose	NonProteinOrNucleicAcidChemical		is present in					rabbits	Organism	milk of;;lactating			NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Effect of reserpine on the lactose , iron and lactoferrin content of the milk of lactating rabbits ) .	manualset1
79706	2	356907	5	NULL	NULL	0	NULL	reserpine	NonProteinOrNucleicAcidChemical		effects		may			statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of reserpine on the lactose , iron and lactoferrin content of the milk of lactating rabbits ) .	manualset1
79707	3	356907	5	NULL	NULL	NULL	NULL	iron	NonProteinOrNucleicAcidChemical		is present in					rabbits	Organism	milk of;;lactating			NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Effect of reserpine on the lactose , iron and lactoferrin content of the milk of lactating rabbits ) .	manualset1
79708	4	356907	5	NULL	NULL	0	NULL	reserpine	NonProteinOrNucleicAcidChemical		effects		may			statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of reserpine on the lactose , iron and lactoferrin content of the milk of lactating rabbits ) .	manualset1
79709	5	356907	5	NULL	NULL	0	NULL	lactoferrin	NonProteinOrNucleicAcidChemical		is present in					rabbits	Organism	milk of;;lactating			NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of reserpine on the lactose , iron and lactoferrin content of the milk of lactating rabbits ) .	manualset1
79710	6	356907	5	NULL	NULL	0	NULL	reserpine	NonProteinOrNucleicAcidChemical		effects		may			statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of reserpine on the lactose , iron and lactoferrin content of the milk of lactating rabbits ) .	manualset1
79711	1	356909	5	NULL	NULL	0	NULL	siRNA	NucleicAcid	transfection of	targets					VEGF gene	Gene				NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of siRNA transfection targeting VEGF gene on proliferation and apoptosis of human breast cancer cells ) .	manualset1
79712	2	356909	5	NULL	NULL	0	NULL	statement 1	Process		effects		may			breast cancer cells	Cell	proliferation of;;human			NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of siRNA transfection targeting VEGF gene on proliferation and apoptosis of human breast cancer cells ) .	manualset1
79713	3	356909	5	NULL	NULL	0	NULL	statement 1	Process		effects		may			breast cancer cells	Cell	apoptosis of;;human			NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of siRNA transfection targeting VEGF gene on proliferation and apoptosis of human breast cancer cells ) .	manualset1
79714	1	356911	5	NULL	NULL	0	NULL	starvation	Process		effects		may			respiratory reactivity	Process				NULL	inbred rats	0	NULL	NULL	NULL	NULL	NULL	( Effect of starvation on respiratory reactivity in inbred rats ) .	manualset1
79722	1	356934	5	NULL	NULL	0	NULL	agents	Chemical		stimulates					histamine H1 receptor	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	( Electrophysiological changes in the state of uterine muscles under the action of agents stimulating histamine H1 and H2 receptors ) .	manualset1
79723	2	356934	5	NULL	NULL	0	NULL	agents	Chemical		stimulates					histamine H2 receptor	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	( Electrophysiological changes in the state of uterine muscles under the action of agents stimulating histamine H1 and H2 receptors ) .	manualset1
79724	3	356934	5	NULL	NULL	0	NULL	statement 1	Process		changes					uterine muscles	BodyPart	state of			NULL		0	NULL	NULL	NULL	NULL	NULL	( Electrophysiological changes in the state of uterine muscles under the action of agents stimulating histamine H1 and H2 receptors ) .	manualset1
79725	4	356934	5	NULL	NULL	0	NULL	statement 2	Process		changes					uterine muscles	BodyPart	state of			NULL		0	NULL	NULL	NULL	NULL	NULL	( Electrophysiological changes in the state of uterine muscles under the action of agents stimulating histamine H1 and H2 receptors ) .	manualset1
79726	1	357033	5	NULL	NULL	0	NULL	pancreatic islets	BodyPart		altered by					autoimmune system	AnatomicalPart				NULL	 diabetic subjects	0	NULL	NULL	NULL	NULL	NULL	( Functional study of pancreatic islets altered by the autoimmune system in diabetic and non-diabetic subjects ) .	manualset1
79727	2	357033	5	NULL	NULL	0	NULL	pancreatic islets	BodyPart		altered by					autoimmune system	AnatomicalPart				NULL	non-diabetic subjects	0	NULL	NULL	NULL	NULL	NULL	( Functional study of pancreatic islets altered by the autoimmune system in diabetic and non-diabetic subjects ) .	manualset1
79728	1	357062	5	NULL	NULL	0	NULL	myocardial calcification	MedicalFinding	severe	leads to					heart failure	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Heart failure due to severe myocardial calcification -- a rare complication after irradiation on the chest wall ) .	manualset1
79729	2	357062	5	NULL	NULL	0	NULL	statement 1	Process		is a type of					rare complication	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	( Heart failure due to severe myocardial calcification -- a rare complication after irradiation on the chest wall ) .	manualset1
79730	3	357062	5	NULL	NULL	0	NULL	statement 1	Process		occurs after					chest wall	BodyPart	irradiation of			NULL		0	NULL	NULL	NULL	NULL	NULL	( Heart failure due to severe myocardial calcification -- a rare complication after irradiation on the chest wall ) .	manualset1
79731	1	357066	5	NULL	NULL	0	NULL	Hemosorption	NonProteinOrNucleicAcidChemical		treats					occlusive arterial diseases	Disease				NULL	legs	0	NULL	NULL	NULL	NULL	NULL	( Hemosorption in the treatment of occlusive arterial diseases of the legs ) .	manualset1
79732	1	357067	5	NULL	NULL	0	NULL	mexamine	NonProteinOrNucleicAcidChemical	hemostatic action of 	plays a role in					acute radiation sickness	Disease	experimental			NULL		0	NULL	NULL	NULL	NULL	NULL	( Hemostatic action of serotonin and mexamine in experimental acute radiation sickness ) .	manualset1
79733	2	357067	5	NULL	NULL	0	NULL	serotonin	Protein	hemostatic action of	plays a role in					acute radiation sickness	Disease	experimental			NULL		0	NULL	NULL	NULL	NULL	NULL	( Hemostatic action of serotonin and mexamine in experimental acute radiation sickness ) .	manualset1
79734	1	357069	5	NULL	NULL	0	NULL	pneumonia	Disease		causes					hepatocellular damage	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	( Hepatocellular damage during pneumonia ) .	manualset1
79735	1	357075	5	NULL	NULL	0	NULL	heparin	NonProteinOrNucleicAcidChemical		release					Histaminase	Protein				NULL	guinea pigs	0	NULL	NULL	NULL	NULL	NULL	( Histaminase release by heparin and protamine in guinea pigs ) .	manualset1
79736	2	357075	5	NULL	NULL	0	NULL	protamine	Protein		release					Histaminase	Protein				NULL	guinea pigs	0	NULL	NULL	NULL	NULL	NULL	( Histaminase release by heparin and protamine in guinea pigs ) .	manualset1
79737	1	357100	5	NULL	NULL	0	NULL	granulocytes	Cell	increase of	leads to					Hyperleukocytosis	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Hyperleukocytosis due to an increase in granulocytes ) .	manualset1
79738	1	357104	5	NULL	NULL	0	NULL	Hypoxidosis	MedicalFinding		causal factor in					skin diseases	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Hypoxidosis as causal factor in skin diseases ) .	manualset1
79826	1	357114	5	NULL	NULL	0	NULL	ICAM-1	Protein		is					intercellular cell adhesion molecule 1	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	( Immunohistologic study of the localization of ICAM-1 ( intercellular cell adhesion molecule 1 ) in alveolar epithelium in the human lung ) .	manualset1
79827	2	357114	5	NULL	NULL	NULL	NULL	ICAM-1	Protein		is localized in					alveolar epithelium	BodyPart				NULL	human lung	NULL	NULL	NULL	NULL	NULL	NULL	( Immunohistologic study of the localization of ICAM-1 ( intercellular cell adhesion molecule 1 ) in alveolar epithelium in the human lung ) .	manualset1
79828	1	357119	5	NULL	NULL	0	NULL	celioscopy	MedicalProcedure		is important for		may be			conjugal sterility	Process	involuntary			NULL		0	NULL	NULL	NULL	NULL	NULL	( Importance of celioscopy in involuntary conjugal sterility ) .	manualset1
79829	1	357120	5	NULL	NULL	0	NULL	intracardiac phonocardiography	MedicalProcedure		is important for		may be			tricuspid insufficiency	Disease	diagnosis of			NULL		0	NULL	NULL	NULL	NULL	NULL	( Importance of intracardiac phonocardiography in the diagnosis of tricuspid insufficiency ) .	manualset1
79830	1	357121	5	NULL	NULL	0	NULL	isoimmunization	MedicalProcedure		is important for		may be			mongoloid idiocy	Disease	pathogenesis of			NULL		0	NULL	NULL	NULL	NULL	NULL	( Importance of isoimmunization in pathogenesis of mongoloid idiocy ) .	manualset1
79875	1	357122	5	NULL	NULL	0	NULL	artificial respiration	MedicalProcedure	prolonged	is important for		may be			closed chest injuries	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	( Importance of prolonged artificial respiration in the treatment of closed chest injuries ) .	manualset1
79880	1	357124	5	NULL	NULL	0	NULL	surfactant system	Chemical		is important for		may be			hyaline membrane	BodyPart	pathogenesis of			NULL		0	NULL	NULL	NULL	NULL	NULL	( Importance of the `` surfactant system '' in the pathogenesis of hyaline membrane in the newborn ) .	manualset1
79887	1	357142	5	NULL	NULL	0	NULL	mammary carcinomas	Disease		increases during					pregnancy	BiologicalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	( Increase of mammary carcinomas during pregnancy and in the lactation period ) .	manualset1
79888	2	357142	5	NULL	NULL	0	NULL	mammary carcinomas	Disease		increases during					lactation period	Time				NULL		0	NULL	NULL	NULL	NULL	NULL	( Increase of mammary carcinomas during pregnancy and in the lactation period ) .	manualset1
79909	1	357147	5	NULL	NULL	NULL	NULL	antigens	Chemical	Individual	serological cause of					fetal injury	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Individual antigens as serological cause of fetal injury and their role in blood transfusion ) .	manualset1
79914	1	357155	5	NULL	NULL	NULL	NULL	dl-propranolol	NonProteinOrNucleicAcidChemical		inhibits					sperm capacitation	BiologicalProcess	guinea pig			NULL	in vitro	NULL	NULL	NULL	NULL	NULL	NULL	( Inhibition of guinea pig sperm capacitation , the acrosome reaction and sperm-egg fusion by dl-propranolol in vitro ) .	manualset1
79915	2	357155	5	NULL	NULL	0	NULL	dl-propranolol	NonProteinOrNucleicAcidChemical		inhibits					acrosome reaction	BiologicalProcess	guinea pig			NULL	in vitro	0	NULL	NULL	NULL	NULL	NULL	( Inhibition of guinea pig sperm capacitation , the acrosome reaction and sperm-egg fusion by dl-propranolol in vitro ) .	manualset1
79916	3	357155	5	NULL	NULL	0	NULL	dl-propranolol	NonProteinOrNucleicAcidChemical		inhibits					sperm-egg fusion	BiologicalProcess	guinea pig			NULL	in vitro	0	NULL	NULL	NULL	NULL	NULL	( Inhibition of guinea pig sperm capacitation , the acrosome reaction and sperm-egg fusion by dl-propranolol in vitro ) .	manualset1
79921	1	357163	5	NULL	NULL	0	NULL	14-3-3beta	GeneOrProtein	segments of	interacts with					PrP	GeneOrProtein				NULL	in vitro	0	NULL	NULL	NULL	NULL	NULL	( Interaction between various 14-3-3beta segments and PrP in vitro ) .	manualset1
79922	1	357165	5	NULL	NULL	0	NULL	androgen	GeneOrProtein		deprived in		intermittently			prostate cancer	Disease	advanced			NULL		0	NULL	NULL	NULL	NULL	NULL	( Intermittent androgen deprivation in advanced prostate cancer : a review ) .	manualset1
79923	1	357171	5	NULL	NULL	0	NULL	Intestinal occlusion	Disease		is caused by					retroperitoneal cysts	MedicalFinding	wolffian			NULL		0	NULL	NULL	NULL	NULL	NULL	( Intestinal occlusion caused by retroperitoneal cysts of wolffian origin ) .	manualset1
79924	1	357173	5	NULL	NULL	0	NULL	Intra uterine asphyxia	MedicalFinding		leads to					stillbirth					NULL		0	NULL	NULL	NULL	NULL	NULL	( Intra uterine asphyxia as a main factor of stillbirth ) .	manualset1
79925	1	357175	5	NULL	NULL	0	NULL	hyaluronic acid	NonProteinOrNucleicAcidChemical	Intra-articular injections of	plays a role in		may			knee osteoarthritis	Disease	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	( Intra-articular injections of hyaluronic acid in the treatment of knee osteoarthritis ) .	manualset1
79926	1	357185	5	NULL	NULL	0	NULL	H1 histone	Protein	phosphorylation of	is involved in					chromosome condensation	BiologicalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	( Involvement of H1 histone phosphorylation in chromosome condensation at mitosis ) .	manualset1
79927	2	357185	5	NULL	NULL	0	NULL	statement 1	Process		occurs during					mitosis	BiologicalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	( Involvement of H1 histone phosphorylation in chromosome condensation at mitosis ) .	manualset1
79928	1	357196	5	NULL	NULL	0	NULL	methotrexate	NonProteinOrNucleicAcidChemical		treats					rheumatic diseases	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Italian consensus on the recommendations about the use of methotrexate for the treatment of rheumatic diseases with a focus on rheumatoid arthritis : results from the `` 3E initiative '' ) .	manualset1
79929	1	357201	5	NULL	NULL	0	NULL	Klimovan injection	MedicalProcedure		is a diagnostic method in					pregnancy	BiologicalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	( KLIMOVAN INJECTION AS A DIAGNOSTIC METHOD IN PREGNANCY ) .	manualset1
79930	1	357202	5	NULL	NULL	0	NULL	Ketamine	NonProteinOrNucleicAcidChemical		is used to treat		may be			status asthmaticus	Disease	severe;;therapy-resistant			NULL		0	NULL	NULL	NULL	NULL	NULL	( Ketamine in the treatment of severe therapy-resistant status asthmaticus ) .	manualset1
79931	1	357209	5	NULL	NULL	0	NULL	prednisone	NonProteinOrNucleicAcidChemical	imbalance of;;dosages of	influence		may			kidney	BodyPart	rejection of			NULL		0	NULL	NULL	NULL	NULL	NULL	( Late kidney rejection : influence of imbalance in prednisone and azathioprine dosages ) .	manualset1
79932	2	357209	5	NULL	NULL	0	NULL	azathioprine	NonProteinOrNucleicAcidChemical	imbalance of;;dosages of	influence		may			kidney	BodyPart	rejection of			NULL		0	NULL	NULL	NULL	NULL	NULL	( Late kidney rejection : influence of imbalance in prednisone and azathioprine dosages ) .	manualset1
79934	1	357221	5	NULL	NULL	0	NULL	PLAC 1	NonProteinOrNucleicAcidChemical		is					pravastatin	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	( Limitation of atherosclerosis in coronary arteries with pravastatin ( PLAC 1 ) ) .	manualset1
79935	2	357221	5	NULL	NULL	0	NULL	pravastatin	NonProteinOrNucleicAcidChemical		limits					atherosclerosis	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Limitation of atherosclerosis in coronary arteries with pravastatin ( PLAC 1 ) ) .	manualset1
79936	3	357221	5	NULL	NULL	0	NULL	statement 2	Process		occurs in					coronary arteries	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	( Limitation of atherosclerosis in coronary arteries with pravastatin ( PLAC 1 ) ) .	manualset1
79937	1	357222	5	NULL	NULL	0	NULL	noradrenaline	NonProteinOrNucleicAcidChemical		limits					noradrenaline	NonProteinOrNucleicAcidChemical	vascular effects of			NULL		0	NULL	NULL	NULL	NULL	NULL	( Limitation of the vascular effects of noradrenaline using noradrenaline itself ) .	manualset1
79938	1	357226	5	NULL	NULL	NULL	NULL	Lipoprotein ( a )	Chemical		is a marker for					coronary disease	Disease	presence of;;severity of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Lipoprotein ( a ) , D-Dimer and apolipoprotein A1 as markers of presence and severity of coronary disease ) .	manualset1
79941	2	357226	5	NULL	NULL	0	NULL	D-Dimer	Chemical		is a marker for					coronary disease	Disease	presence of;;severity of			NULL		0	NULL	NULL	NULL	NULL	NULL	( Lipoprotein ( a ) , D-Dimer and apolipoprotein A1 as markers of presence and severity of coronary disease ) .	manualset1
79943	3	357226	5	NULL	NULL	0	NULL	apolipoprotein A1	Protein		is a marker for					coronary disease	Disease	presence of;;severity of			NULL		0	NULL	NULL	NULL	NULL	NULL	( Lipoprotein ( a ) , D-Dimer and apolipoprotein A1 as markers of presence and severity of coronary disease ) .	manualset1
79990	1	357251	5	NULL	NULL	0	NULL	hemoptysis	Disease		is caused by					bronchial aneurysm	MedicalFinding	disruption of			NULL		0	NULL	NULL	NULL	NULL	NULL	( Massive hemoptysis caused by disruption of a bronchial aneurysm diagnosed by microscopic examination of the resected lung ) .	manualset1
79991	1	357260	5	NULL	NULL	0	NULL	enterotoxic staphylococci	Organism		causes					food poisoning	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Medico-legal considerations on a case of food poisoning due to enterotoxic staphylococci ) .	manualset1
79992	1	357268	5	NULL	NULL	0	NULL	Micafungin	NonProteinOrNucleicAcidChemical		is used to treat					invasive mycoses	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Micafungin , a new candin for the treatment of invasive mycoses ) .	manualset1
79993	1	357390	5	NULL	NULL	0	NULL	injuries	MedicalFinding	indirect	causes					Optic atrophy	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Optic atrophy caused by indirect injuries ) .	manualset1
79994	1	357424	5	NULL	NULL	0	NULL	Ca2 +	Chemical		influx into		passively			sarcoplasmic reticulum	BodyPart	vesicles of			NULL		0	NULL	NULL	NULL	NULL	NULL	( Passive Ca2 + influx into vesicles of the sarcoplasmic reticulum , modified by succinic anhydride ) .	manualset1
79995	2	357424	5	NULL	NULL	0	NULL	succinic anhydride	NonProteinOrNucleicAcidChemical		modifies					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	( Passive Ca2 + influx into vesicles of the sarcoplasmic reticulum , modified by succinic anhydride ) .	manualset1
80080	1	357454	5	NULL	NULL	0	NULL	aldosterone	NonProteinOrNucleicAcidChemical		is a type of					Plasma mineralocorticoids	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	( Plasma mineralocorticoids -- aldosterone and desoxycorticosterone -- in patients with `` low-renin `` arterial hypertension ) .	manualset1
80081	2	357454	5	NULL	NULL	0	NULL	desoxycorticosterone	NonProteinOrNucleicAcidChemical		is a type of					Plasma mineralocorticoids	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	( Plasma mineralocorticoids -- aldosterone and desoxycorticosterone -- in patients with `` low-renin `` arterial hypertension ) .	manualset1
80082	1	357458	5	NULL	NULL	0	NULL	Pneumocystis carinii pneumopathy	Disease		occurs in					rheumatoid polyarthritis	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Pneumocystis carinii pneumopathy in rheumatoid polyarthritis treated by methotrexate in a patient with pulmonary asbestosis ) .	manualset1
80083	2	357458	5	NULL	NULL	0	NULL	methotrexate	NonProteinOrNucleicAcidChemical		treats					statement 1	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Pneumocystis carinii pneumopathy in rheumatoid polyarthritis treated by methotrexate in a patient with pulmonary asbestosis ) .	manualset1
80084	3	357458	5	NULL	NULL	0	NULL	statement 2	Process		occurs in					pulmonary asbestosis patient					NULL		0	NULL	NULL	NULL	NULL	NULL	( Pneumocystis carinii pneumopathy in rheumatoid polyarthritis treated by methotrexate in a patient with pulmonary asbestosis ) .	manualset1
80085	1	357556	5	NULL	NULL	0	NULL	radiation	EnvironmentalFactor		induce					injuries	MedicalFinding				NULL	children	0	NULL	NULL	NULL	NULL	NULL	( Radiation-induced injuries following roentgenotherapy of angiomas in children depending on the technic of radiation use ) .	manualset1
80086	2	357556	5	NULL	NULL	0	NULL	statement 1	Process		follows					angiomas	Disease	roentgenotherapy of			NULL	children	0	NULL	NULL	NULL	NULL	NULL	( Radiation-induced injuries following roentgenotherapy of angiomas in children depending on the technic of radiation use ) .	manualset1
80087	3	357556	5	NULL	NULL	NULL	NULL	statement 1	Process		depends on					raditaion	LaboratoryExperimentalFactor	technic of;;use of			NULL	children	NULL	NULL	NULL	NULL	NULL	NULL	( Radiation-induced injuries following roentgenotherapy of angiomas in children depending on the technic of radiation use ) .	manualset1
80088	1	357557	5	NULL	NULL	0	NULL	 Radioactive iodine treatment 	MedicalProcedure		is used to treat					hyperthyroidism	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Radioactive iodine treatment of hyperthyroidism associated with diabetes ) .	manualset1
80089	2	357557	5	NULL	NULL	0	NULL	statement 1	Process		is associated with					diabetes	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Radioactive iodine treatment of hyperthyroidism associated with diabetes ) .	manualset1
80090	1	357562	5	NULL	NULL	0	NULL	Raloxifene	NonProteinOrNucleicAcidChemical		is a modulator of		selective			estrogen receptors	GeneOrProtein				NULL		0	NULL	NULL	NULL	NULL	NULL	( Raloxifene : a selective modulator of estrogen receptors ) .	manualset1
80091	1	357575	5	NULL	NULL	0	NULL	hypotensive medication	MedicalProcedure		reduces the risk of					stroke	Disease	recurrence of			NULL		0	NULL	NULL	NULL	NULL	NULL	( Reduced risk of stroke recurrence due to hypotensive medication , irrespective of the initial blood pressure ) .	manualset1
80092	2	357575	5	NULL	NULL	0	NULL	statement 1	Process		irrespective of					blood pressure	EnvironmentalFactor	initial			NULL		0	NULL	NULL	NULL	NULL	NULL	( Reduced risk of stroke recurrence due to hypotensive medication , irrespective of the initial blood pressure ) .	manualset1
80093	2	357576	5	NULL	NULL	NULL	NULL	statement 1	Process		undergoes					reduction	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Reduction of the functional activity of the calcium pump of the sarcoplasmic reticulum of skeletal muscles in response to cold ) .	manualset1
80094	3	357576	5	NULL	NULL	NULL	NULL	statement 2	Process		in response to					cold	EnvironmentalFactor				NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Reduction of the functional activity of the calcium pump of the sarcoplasmic reticulum of skeletal muscles in response to cold ) .	manualset1
80095	1	357576	5	NULL	NULL	0	NULL	calcium pump	BiologicalProcess		is active in		functionally			sarcoplasmic reticulum	BodyPart				NULL	skeletal muscles	0	NULL	NULL	NULL	NULL	NULL	( Reduction of the functional activity of the calcium pump of the sarcoplasmic reticulum of skeletal muscles in response to cold ) .	manualset1
80096	1	357590	5	NULL	NULL	0	NULL	 vincaleukoblastine	NonProteinOrNucleicAcidChemical		treats					malignant cutaneous reticulosis	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Remarkable action of vincaleukoblastine in the treatment of a case of malignant cutaneous reticulosis ) .	manualset1
80097	1	357595	5	NULL	NULL	0	NULL	angioplasty	MedicalProcedure		is not essential for					Renovascular hypertension	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Renovascular hypertension : angioplasty need not be essential ) .	manualset1
80098	1	357598	5	NULL	NULL	0	NULL	mandibular condyle	BodyPart	high fractures of;;neck of	leads to					mandibular condyle	BodyPart	dislocation of			NULL		0	NULL	NULL	NULL	NULL	NULL	( Replantation as a method of treating high fractures of the neck of the mandibular condyle with dislocation of the articular head ) .	manualset1
80099	2	357598	5	NULL	NULL	0	NULL	Replantation	MedicalProcedure		is used to treat					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	( Replantation as a method of treating high fractures of the neck of the mandibular condyle with dislocation of the articular head ) .	manualset1
80100	1	357604	5	NULL	NULL	0	NULL	Cd2 +	Chemical	soil	is absorbed by					perennial ryegrass	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	( Research on the relevance of earthworms inducing soil Cd2 + absorbed by perennial ryegrass ) .	manualset1
80101	1	357626	5	NULL	NULL	NULL	NULL	apoptosis	BiologicalProcess	renal tubular cells	is induced by					post asphyxial serum	CellComponent	neonate			NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Role of Omi/HtrA2 in renal tubular cells apoptosis induced by post asphyxial serum of neonate ) .	manualset1
80102	1	357630	5	NULL	NULL	NULL	NULL	epithelium	BodyPart		transition to					mesenchyma	BodyPart				NULL	human peritoneal mesothelial cells	NULL	NULL	NULL	NULL	NULL	NULL	( Role of galectin-1 on epithelial-to-mesenchymal transition induced by high glucose peritoneal dialysate in human peritoneal mesothelial cells ) .	manualset1
80104	2	357630	5	NULL	NULL	0	NULL	glucose peritoneal dialysate	NonProteinOrNucleicAcidChemical	high	induce					statement 1					NULL	human peritoneal mesothelial cells	0	NULL	NULL	NULL	NULL	NULL	( Role of galectin-1 on epithelial-to-mesenchymal transition induced by high glucose peritoneal dialysate in human peritoneal mesothelial cells ) .	manualset1
80105	1	357639	5	NULL	NULL	0	NULL	Rubiaceae	Organism		is an important component of					medicine	Chemical	ayurvedic system of			NULL		0	NULL	NULL	NULL	NULL	NULL	( Rubiaceae ) is an important component of the ayurvedic system of medicine .	manualset1
80106	1	357643	5	NULL	NULL	0	NULL	abdominal wall	BodyPart	Sarcoma of	is ruptured during					labor	BiologicalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	( Sarcoma of the abdominal wall ruptured during labor ) .	manualset1
80107	1	357650	5	NULL	NULL	0	NULL	Neisseria gonorrhoeae	Organism		is sensitive to					spectinomycin	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	( Sensitivity of Neisseria gonorrhoeae to spectinomycin ) .	manualset1
80108	1	357651	5	NULL	NULL	0	NULL	ectoparasites	Organism	chicken	is sensitive to					methylbromfenvinphos	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	( Sensitivity of ectoparasites of chickens to methylbromfenvinphos ( Polwet 5 and Polwet 20 ) .	manualset1
80109	1	357659	5	NULL	NULL	NULL	NULL	encysted purulent pleurisy	Disease		leads to					pulmonary tuberculosis	Disease	severe			NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Severe pulmonary tuberculosis after encysted purulent pleurisy ) .	manualset1
80110	1	357666	5	NULL	NULL	0	NULL	fibrosis	MedicalFinding		is developed in					systemic scleroderma	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Significance of estradiol in the development of fibrosis in systemic scleroderma ( bases of sexual predisposition to the disease ) ) .	manualset1
80136	1	357679	5	NULL	NULL	0	NULL	Soft-tissue	BodyPart		changes in					metacarpal area	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	( Soft-tissue changes in the metacarpal area in chronic polyarthritis ) .	manualset1
80137	2	357679	5	NULL	NULL	0	NULL	statement 1	Process		occurs in					chronic polyarthritis	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Soft-tissue changes in the metacarpal area in chronic polyarthritis ) .	manualset1
80138	1	357682	5	NULL	NULL	0	NULL	streptomycin	NonProteinOrNucleicAcidChemical		changes					antigenic complex	Chemical	Bacillus anthracis			NULL		0	NULL	NULL	NULL	NULL	NULL	( Some changes in the antigenic complex of Bacillus anthracis under the action of streptomycin ) .	manualset1
80139	1	357693	5	NULL	NULL	0	NULL	granuloma 	MedicalFinding	spermatozoal	causes		possibly			hydrocele	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Spermatozoal granuloma as a possible cause of hydrocele ) .	manualset1
80140	1	357695	5	NULL	NULL	NULL	NULL	ureteric tumor	Disease	metastatic 	ruptures		spontaneously			ureter	BodyPart				NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Spontaneous rupture of the ureter caused by metastatic ureteric tumor : a case report ) .	manualset1
80141	1	357696	5	NULL	NULL	NULL	NULL	excitation	BiologicalProcess		spreads from					ventromedial hypothalamus	BodyPart	brain			NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Spread of excitation from the ventromedial hypothalamus to the limbic-reticular structure of the brain ) .	manualset1
80142	2	357696	5	NULL	NULL	0	NULL	excitation	BiologicalProcess		spreads to					limbic-reticular structure	BodyPart	brain			NULL		0	NULL	NULL	NULL	NULL	NULL	( Spread of excitation from the ventromedial hypothalamus to the limbic-reticular structure of the brain ) .	manualset1
80143	3	357696	5	NULL	NULL	0	NULL	statement 1	Process		occurs simultaneously with					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	( Spread of excitation from the ventromedial hypothalamus to the limbic-reticular structure of the brain ) .	manualset1
80144	1	357709	5	NULL	NULL	0	NULL	Stiff man syndrome	Disease		is also known as					Moersch and Woltman syndrome	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Stiff man syndrome ( Moersch and Woltman syndrome ) .	manualset1
80145	1	357712	5	NULL	NULL	0	NULL	( Strept ) avidins	Protein		is a type of					exceptionally stable proteins	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	( Strept ) avidins are also exceptionally stable proteins .	manualset1
80146	1	357718	5	NULL	NULL	0	NULL	baicalin	NonProteinOrNucleicAcidChemical	metabolites of	is present in					urine	Chemical	human			NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on metabolites of baicalin in human urine ) .	manualset1
80823	1	357734	5	NULL	NULL	0	NULL	LDL receptors	Protein		is present in					non-parenchymal cells	Cell	liver			NULL		0	NULL	NULL	NULL	NULL	NULL	( Study on LDL receptors of liver non-parenchymal cells in hypertriglyceridemic rats induced by high carbohydrate diet ) .	manualset1
80824	2	357734	5	NULL	NULL	0	NULL	statement 1	Process		is present in					rat	Organism	hypertriglyceridemic			NULL		0	NULL	NULL	NULL	NULL	NULL	( Study on LDL receptors of liver non-parenchymal cells in hypertriglyceridemic rats induced by high carbohydrate diet ) .	manualset1
80825	3	357734	5	NULL	NULL	0	NULL	high carbohydrate diet	Food		induce					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	( Study on LDL receptors of liver non-parenchymal cells in hypertriglyceridemic rats induced by high carbohydrate diet ) .	manualset1
80826	1	357735	5	NULL	NULL	0	NULL	572 C/G	Gene		is a type of					interleukin 6 gene	Gene				NULL		0	NULL	NULL	NULL	NULL	NULL	( Study on linkage between polymorphism of interleukin 6 gene -572 C/G and susceptibility to myocardial infarction ) .	manualset1
80827	2	357735	5	NULL	NULL	NULL	NULL	572 C/G	Gene	polymorphism of	is linked to		may be			myocardial infarction	Process	susceptibility of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Study on linkage between polymorphism of interleukin 6 gene -572 C/G and susceptibility to myocardial infarction ) .	manualset1
80829	1	357737	5	NULL	NULL	0	NULL	Subacute septic endocarditis	Disease		is complicated by					vessels	OrganismPart	aneurysm of;;major			NULL		0	NULL	NULL	NULL	NULL	NULL	( Subacute septic endocarditis complicated by an aneurysm of the major vessels ) .	manualset1
80830	1	357738	5	NULL	NULL	0	NULL	Subclinical pulmonary dysfunction	MedicalFinding		is a complication of		probably			diabetes	Disease	unrecognized			NULL		0	NULL	NULL	NULL	NULL	NULL	( Subclinical pulmonary dysfunction : an unrecognized diabetes complication ? ) .	manualset1
80831	1	357742	5	NULL	NULL	NULL	NULL	cystoid macular edema	Disease		is treated with		successfully			etanercept	NonProteinOrNucleicAcidChemical				NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Successful treatment of cystoid macular edema with etanercept in a patient with rheumatoid arthritis associated panuveitis ) .	manualset1
80832	2	357742	5	NULL	NULL	0	NULL	statement 1	Process		occurs in					panuveitis patients	PersonGroup				NULL		0	NULL	NULL	NULL	NULL	NULL	( Successful treatment of cystoid macular edema with etanercept in a patient with rheumatoid arthritis associated panuveitis ) .	manualset1
80833	3	357742	5	NULL	NULL	0	NULL	panuveitis	Disease		is associated with					rheumatoid arthritis	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Successful treatment of cystoid macular edema with etanercept in a patient with rheumatoid arthritis associated panuveitis ) .	manualset1
80838	1	357743	5	NULL	NULL	0	NULL	pituitary-adrenal axis	Process		is suppressed by					triamcinolone acetonide	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	( Suppression of pituitary-adrenal axis by triamcinolone acetonide in asthmatics ) .	manualset1
80839	2	357743	5	NULL	NULL	0	NULL	statement 1	Process		occurs in					asthmatics	PersonGroup				NULL		0	NULL	NULL	NULL	NULL	NULL	( Suppression of pituitary-adrenal axis by triamcinolone acetonide in asthmatics ) .	manualset1
80844	1	357750	5	NULL	NULL	0	NULL	intrahepatic biliary stones	MedicalFinding		is treated with					surgery	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	( Surgical treatment of intrahepatic biliary stones ) .	manualset1
80850	1	357751	5	NULL	NULL	0	NULL	malignant neoplasms	Disease		occurs in					pancreatoduodenal zone	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	( Surgical treatment of malignant neoplasms of the pancreatoduodenal zone ) .	manualset1
80851	2	357751	5	NULL	NULL	0	NULL	statement 1	Process		is treated with					surgery	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	( Surgical treatment of malignant neoplasms of the pancreatoduodenal zone ) .	manualset1
80852	1	357752	5	NULL	NULL	0	NULL	myocardial infarct	Disease		is treated with					surgery	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	( Surgical treatment of myocardial infarct in complications .	manualset1
80853	1	357753	5	NULL	NULL	0	NULL	intramedullary tumors	Disease		occurs in					neck	BodyPart	upper			NULL		0	NULL	NULL	NULL	NULL	NULL	( Surgically treated case of intramedullary tumors of the upper neck witn an interesting postoperative course ) .	manualset1
80854	2	357753	5	NULL	NULL	0	NULL	statement 1	Process		is treated with					surgery	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	( Surgically treated case of intramedullary tumors of the upper neck witn an interesting postoperative course ) .	manualset1
80855	1	357756	5	NULL	NULL	0	NULL	Legionella pneumonia	Disease		shows					KL-6	Protein	high level of;;serum			NULL		0	NULL	NULL	NULL	NULL	NULL	( Surviving case of Legionella pneumonia showing a high level of serum KL-6 and complicated with rhabdomyolysis ) .	manualset1
80856	1	357757	5	NULL	NULL	0	NULL	Pseudomonas species	Organism		susceptibile to					aminoglycosides	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	( Susceptibilities of Pseudomonas species to aminoglycosides and tetracyclines ) .	manualset1
80857	2	357757	5	NULL	NULL	0	NULL	Pseudomonas species	Organism		susceptibile to					tetracyclines	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	( Susceptibilities of Pseudomonas species to aminoglycosides and tetracyclines ) .	manualset1
80858	1	357760	5	NULL	NULL	0	NULL	THAM citrate	NonProteinOrNucleicAcidChemical	oral administration of	treats					renal acidosis	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Symptomatic treatment of renal acidosis by oral administration of THAM citrate ) .	manualset1
80859	1	357762	5	NULL	NULL	0	NULL	testicular cells	Cell		express					Fas ligand	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	( Synergistic protective effect of testicular cells expressing Fas ligand and cyclosporine A on the survival of islet allografts ) .	manualset1
80860	2	357762	5	NULL	NULL	0	NULL	statement 1	Process		effects		protective			islet allografts	BodyPart	survival of			NULL		0	NULL	NULL	NULL	NULL	NULL	( Synergistic protective effect of testicular cells expressing Fas ligand and cyclosporine A on the survival of islet allografts ) .	manualset1
80861	3	357762	5	NULL	NULL	0	NULL	cyclosporine A	NonProteinOrNucleicAcidChemical		effects		protective			islet allografts	BodyPart	survival of			NULL		0	NULL	NULL	NULL	NULL	NULL	( Synergistic protective effect of testicular cells expressing Fas ligand and cyclosporine A on the survival of islet allografts ) .	manualset1
80862	4	357762	5	NULL	NULL	0	NULL	statement 2	Process		synergistic to					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	( Synergistic protective effect of testicular cells expressing Fas ligand and cyclosporine A on the survival of islet allografts ) .	manualset1
80863	1	357765	5	NULL	NULL	0	NULL	quinolines	NonProteinOrNucleicAcidChemical		is synthesised from					safrole	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	( Synthesis of quinolines from safrole ) .	manualset1
81122	1	357771	5	NULL	NULL	NULL	NULL	Chondroitin Sulphuric Acid	NonProteinOrNucleicAcidChemical		protective agent for					corneal transparency	BiologicalProcess				NULL		NULL	NULL	NULL	NULL	NULL	NULL	( THE EFFECT OF CHONDROITIN SULFURIC ACID USED AS PROTECTIVE AGENT FOR CORNEAL TRANSPARENCY DURING THE OPERATION OF RETINAL DETACHMENT ) .	manualset1
81123	2	357771	5	NULL	NULL	0	NULL	statement 1	Process		during					retinal detachment	Disease	operation of			NULL		0	NULL	NULL	NULL	NULL	NULL	( THE EFFECT OF CHONDROITIN SULFURIC ACID USED AS PROTECTIVE AGENT FOR CORNEAL TRANSPARENCY DURING THE OPERATION OF RETINAL DETACHMENT ) .	manualset1
81124	1	357777	5	NULL	NULL	0	NULL	TachoSil	Chemical		is used in					urologic surgery	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	( TachoSil : the value of its use in urologic surgery .	manualset1
81125	1	357792	5	NULL	NULL	0	NULL	A771726	NonProteinOrNucleicAcidChemical		is a metabolite of		active			leflunomide	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	( The active metabolite of leflunomide A771726 inhibits proliferation and collagen synthesis of hepatic stellate cell ) .	manualset1
81126	2	357792	5	NULL	NULL	0	NULL	A771726	NonProteinOrNucleicAcidChemical		inhibits					hepatic stellate cell	Cell	proliferation of			NULL		0	NULL	NULL	NULL	NULL	NULL	( The active metabolite of leflunomide A771726 inhibits proliferation and collagen synthesis of hepatic stellate cell ) .	manualset1
81127	3	357792	5	NULL	NULL	0	NULL	collagen	Protein		is synthesised by					hepatic stellate cell	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	( The active metabolite of leflunomide A771726 inhibits proliferation and collagen synthesis of hepatic stellate cell ) .	manualset1
81128	4	357792	5	NULL	NULL	0	NULL	A771726	NonProteinOrNucleicAcidChemical		inhibits					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	( The active metabolite of leflunomide A771726 inhibits proliferation and collagen synthesis of hepatic stellate cell ) .	manualset1
81130	1	357793	5	NULL	NULL	0	NULL	lipid peroxidation	BiologicalProcess		is active in					small intestine	BodyPart	mucosa of;;rat			NULL		0	NULL	NULL	NULL	NULL	NULL	( The activity of the lipid peroxidation processes in the mucosa of the rat small intestine and its morphofunctional state under acute irradiation and the administration of combined preparations created on a base of highly dispersed silica ) .	manualset1
81137	1	357795	5	NULL	NULL	0	NULL	hyaluronidase	Protein		is a type of					antialgesic	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	( The antialgesic action of hyaluronidase in the treatment of medicinal apical parodontitis after filling of the canal ) .	manualset1
81138	2	357795	5	NULL	NULL	0	NULL	statement 1	Protein		is used to treat					medicinal apical parodontitis	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( The antialgesic action of hyaluronidase in the treatment of medicinal apical parodontitis after filling of the canal ) .	manualset1
81139	1	357839	5	NULL	NULL	0	NULL	cefozopran	NonProteinOrNucleicAcidChemical		is a type of					antibacterial	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	( The in vitro antibacterial activity of cefozopran against clinically isolated bacteria ) .	manualset1
81140	2	357839	5	NULL	NULL	0	NULL	cefozopran	NonProteinOrNucleicAcidChemical		acts against					bacteria	Organism	clinically isolated			NULL	in vitro	0	NULL	NULL	NULL	NULL	NULL	( The in vitro antibacterial activity of cefozopran against clinically isolated bacteria ) .	manualset1
81143	1	357843	5	NULL	NULL	0	NULL	enteral feeding	MedicalProcedure	early postoperative	performed through		possibly			 jejunal tube	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	( The jejunal tube : a possibility for early postoperative enteral feeding ) .	manualset1
81144	2	357846	5	NULL	NULL	0	NULL	glucan	NonProteinOrNucleicAcidChemical		induce					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	( The mechanism of glucan-induced agglutination of Actinomyces viscosus ( author 's transl ) ) .	manualset1
81145	1	357846	5	NULL	NULL	NULL	NULL	Actinomyces viscosus	Organism		undergoes					agglutination	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The mechanism of glucan-induced agglutination of Actinomyces viscosus ( author 's transl ) ) .	manualset1
81147	1	357857	5	NULL	NULL	0	NULL	phosphoenolpyruvate	NonProteinOrNucleicAcidChemical		is present in					milk	Food				NULL		0	NULL	NULL	NULL	NULL	NULL	( The phosphoenolpyruvate content of milk as an indicator of the energy balance of the dairy cow ( short communication ) ) .	manualset1
81148	2	357857	5	NULL	NULL	0	NULL	phosphoenolpyruvate	NonProteinOrNucleicAcidChemical		is an indicator of					energy balance	Process				NULL	dairy cow	0	NULL	NULL	NULL	NULL	NULL	( The phosphoenolpyruvate content of milk as an indicator of the energy balance of the dairy cow ( short communication ) ) .	manualset1
81149	1	357870	5	NULL	NULL	0	NULL	nitric oxide	NonProteinOrNucleicAcidChemical		released from					nitroso compounds	NonProteinOrNucleicAcidChemical	organic			NULL	body of animals	0	NULL	NULL	NULL	NULL	NULL	( The release of nitric oxide from organic nitroso compounds in the body of animals ) .	manualset1
81150	1	357882	5	NULL	NULL	0	NULL	Nassarius sp	Organism		causes					poisoning	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	( The study of poisoning caused by Nassa ( Nassarius sp . )	manualset1
81254	1	357910	5	NULL	NULL	0	NULL	Thoracic pain	MedicalFinding		is caused by					coronary insufficiency	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Thoracic pain caused by coronary insufficiency ) .	manualset1
81255	1	357915	5	NULL	NULL	0	NULL	Thrombendarterectomy	MedicalProcedure		prevents		possibly			cerebrovascular insult	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Thrombendarterectomy of the carotid artery in the prevention of cerebrovascular insult ) .	manualset1
81256	2	357915	5	NULL	NULL	0	NULL	statement 1	Process		occurs in					carotid artery	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	( Thrombendarterectomy of the carotid artery in the prevention of cerebrovascular insult ) .	manualset1
81259	1	357918	5	NULL	NULL	0	NULL	Thrombosis	Disease		occurs at 					aortic aneurysm	MedicalFinding	abdominal			NULL		0	NULL	NULL	NULL	NULL	NULL	( Thrombosis at the site of abdominal aortic aneurysm with repeated myocardial infarction ) .	manualset1
81260	2	357918	5	NULL	NULL	0	NULL	statement 1	Process		occurs with					myocardial infarction	Disease	repeated			NULL		0	NULL	NULL	NULL	NULL	NULL	( Thrombosis at the site of abdominal aortic aneurysm with repeated myocardial infarction ) .	manualset1
81261	1	357919	5	NULL	NULL	0	NULL	Thrombotic changes	BiologicalProcess		occurs in					hemostasis	BiologicalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	( Thrombotic changes in hemostasis following streptokinase therapy in myocardial infarct ) .	manualset1
81262	2	357919	5	NULL	NULL	0	NULL	statement 1	Process		occurs following					streptokinase therapy	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	( Thrombotic changes in hemostasis following streptokinase therapy in myocardial infarct ) .	manualset1
81263	3	357919	5	NULL	NULL	0	NULL	statement 2	Process		occurs in					myocardial infarct	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Thrombotic changes in hemostasis following streptokinase therapy in myocardial infarct ) .	manualset1
81264	1	357947	5	NULL	NULL	0	NULL	mithramycin	NonProteinOrNucleicAcidChemical		treats					hypercalcemia	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Treatment of hypercalcemia with mithramycin ) .	manualset1
81265	1	357949	5	NULL	NULL	0	NULL	varicose ulcers	Disease	leg	is treated with					dura mater	BodyPart	xenogenic			NULL		0	NULL	NULL	NULL	NULL	NULL	( Treatment of varicose ulcers of the leg with xenogenic dura mater of the animal ) .	manualset1
81266	1	357955	5	NULL	NULL	0	NULL	streptococcal endocarditis lenta	Disease		is treated by					penicillin V	NonProteinOrNucleicAcidChemical	oral			NULL		0	NULL	NULL	NULL	NULL	NULL	( Two cases of streptococcal endocarditis lenta treated by oral penicillin V ) .	manualset1
81267	1	357959	5	NULL	NULL	0	NULL	unilateral nerve lesion	MedicalFinding	surgical;;recurrent	is an indication for					tracheotomy	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	( UNILATERAL SURGICAL RECURRENT NERVE LESION AS AN INDICATION FOR TRACHEOTOMY ) .	manualset1
81269	1	357968	5	NULL	NULL	0	NULL	adrenergic beta blockaders	NonProteinOrNucleicAcidChemical		is used in					thyrotoxicosis	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Use of adrenergic beta blockaders in thyrotoxicosis and hypothyroidism ) .	manualset1
81270	2	357968	5	NULL	NULL	0	NULL	adrenergic beta blockaders	NonProteinOrNucleicAcidChemical		is used in					hypothyroidism	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Use of adrenergic beta blockaders in thyrotoxicosis and hypothyroidism ) .	manualset1
81268	1	357969	5	NULL	NULL	0	NULL	immunoglobulin	Protein	high dose;;intravenous	is used in					neurologic disease	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	( Use of high dose intravenous immunoglobulin in neurologic disease ) .	manualset1
81280	1	357975	5	NULL	NULL	0	NULL	arterial infusion chemotherapy	MedicalProcedure	continuous	useful for					residual hepatocellular carcinoma	Disease	post operative;;multiple recurrence			NULL		0	NULL	NULL	NULL	NULL	NULL	( Usefulness of continuous arterial infusion chemotherapy for post operative multiple recurrence and residual hepatocellular carcinoma ) .	manualset1
81496	1	357979	5	NULL	NULL	0	NULL	V-osteotomy	MedicalProcedure		corrects					popliteal fossa contractures	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	( V-osteotomy for the correction of popliteal fossa contractures in spina bifida children ) .	manualset1
81497	2	357979	5	NULL	NULL	0	NULL	popliteal fossa contractures	MedicalFinding		occurs in					spina bifida children	PersonGroup				NULL		0	NULL	NULL	NULL	NULL	NULL	( V-osteotomy for the correction of popliteal fossa contractures in spina bifida children ) .	manualset1
81499	1	357983	5	NULL	NULL	0	NULL	multidetector computed tomography	MedicalProcedureOrDevice		is used in					arterio-venous fistula	Disease	assessment of			NULL		0	NULL	NULL	NULL	NULL	NULL	( Value of multidetector computed tomography and digital subtraction angiography in assessment of arterio-venous fistula for hemodialysis -- own experiences ) .	manualset1
81500	2	357983	5	NULL	NULL	0	NULL	digital subtraction angiography	MedicalProcedureOrDevice		is used in					arterio-venous fistula	Disease	assessment of			NULL		0	NULL	NULL	NULL	NULL	NULL	( Value of multidetector computed tomography and digital subtraction angiography in assessment of arterio-venous fistula for hemodialysis -- own experiences ) .	manualset1
81501	3	357983	5	NULL	NULL	0	NULL	statement 1	Process		is required for					hemodialysis	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	( Value of multidetector computed tomography and digital subtraction angiography in assessment of arterio-venous fistula for hemodialysis -- own experiences ) .	manualset1
81502	4	357983	5	NULL	NULL	0	NULL	statement 2	Process		is required for					hemodialysis	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	( Value of multidetector computed tomography and digital subtraction angiography in assessment of arterio-venous fistula for hemodialysis -- own experiences ) .	manualset1
81498	1	357984	5	NULL	NULL	0	NULL	nuclear magnetic resonance tomography	MedicalProcedureOrDevice		is used in					infrarenal abdominal aortic aneurysms	Disease	diagnosis of			NULL		0	NULL	NULL	NULL	NULL	NULL	( Value of nuclear magnetic resonance tomography in diagnosis of infrarenal abdominal aortic aneurysms .	manualset1
81505	1	357996	5	NULL	NULL	0	NULL	Vesicostomy	MedicalProcedure		is a type of					temporary urinary diversion	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	( Vesicostomy : a temporary urinary diversion in childhood ) .	manualset1
81511	2	357996	5	NULL	NULL	0	NULL	statement 1	Process		is performed during					childhood	Time				NULL		0	NULL	NULL	NULL	NULL	NULL	( Vesicostomy : a temporary urinary diversion in childhood ) .	manualset1
81520	1	358000	5	NULL	NULL	0	NULL	Visceral leishmaniasis	Disease		is associated with					cutaneous lesions	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	( Visceral leishmaniasis associated with cutaneous lesions ) .	manualset1
81527	2	358001	5	NULL	NULL	0	NULL	Voluminous solitary non-parasitic cyst	MedicalFinding	liver	is treated with					statement 1	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	( Voluminous solitary non-parasitic cyst of the liver treated with marsupialization and following fistulo-entero-anastomosis ) .	manualset1
81528	1	358001	5	NULL	NULL	0	NULL	marsupialization	MedicalProcedure		is followed by					fistulo-entero-anastomosis	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	( Voluminous solitary non-parasitic cyst of the liver treated with marsupialization and following fistulo-entero-anastomosis ) .	manualset1
81565	1	358030	5	NULL	NULL	NULL	NULL	gI	Protein	deletion of	does not affect			cytoplasmic tail		gE	Protein	intracellular transport of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	( i ) Deletion of the cytoplasmic tail , the transmembrane region plus the C-terminal half of the ectodomain of gI , does not affect intracellular transport of gE .	manualset1
81567	2	358030	5	NULL	NULL	NULL	NULL	gI	Protein	deletion of	does not affect			transmembrane region		gE	Protein	intracellular transport of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	( i ) Deletion of the cytoplasmic tail , the transmembrane region plus the C-terminal half of the ectodomain of gI , does not affect intracellular transport of gE .	manualset1
81569	3	358030	5	NULL	NULL	0	NULL	gI	Protein		is deleted from			C-terminal half		gI	Protein		ectodomain		NULL		0	NULL	NULL	NULL	NULL	NULL	( i ) Deletion of the cytoplasmic tail , the transmembrane region plus the C-terminal half of the ectodomain of gI , does not affect intracellular transport of gE .	manualset1
81570	4	358030	5	NULL	NULL	0	NULL	statement 3	Process		does not affect					gE	Protein	intracellular transport of			NULL		0	NULL	NULL	NULL	NULL	NULL	( i ) Deletion of the cytoplasmic tail , the transmembrane region plus the C-terminal half of the ectodomain of gI , does not affect intracellular transport of gE .	manualset1
81571	1	358031	5	NULL	NULL	0	NULL	virus	Organism	initial;;asymptomatic;;reversible activation of	is judged by					inclusion bearing cells	Cell	presence of			NULL	urine	0	NULL	NULL	NULL	NULL	NULL	( i ) Initial , asymptomatic and reversible activation of the virus , judged by the presence of inclusion bearing cells in the urine .	manualset1
81583	1	358032	5	NULL	NULL	0	NULL	L-NAME	NonProteinOrNucleicAcidChemical		is					 N omega-nitro-L-arginine methyl ester	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	( ii ) The nitric oxide synthase inhibitor N omega-nitro-L-arginine methyl ester ( L-NAME , 100 microM ) did not modulate 5-HT-initiated contractions at either level of PO2 .	manualset1
81584	2	358032	5	NULL	NULL	0	NULL	L-NAME	NonProteinOrNucleicAcidChemical		is an inhibitor of					nitric oxide synthase	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	( ii ) The nitric oxide synthase inhibitor N omega-nitro-L-arginine methyl ester ( L-NAME , 100 microM ) did not modulate 5-HT-initiated contractions at either level of PO2 .	manualset1
81585	3	358032	5	NULL	NULL	0	NULL	contractions	Process		initiated by					5-HT	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	( ii ) The nitric oxide synthase inhibitor N omega-nitro-L-arginine methyl ester ( L-NAME , 100 microM ) did not modulate 5-HT-initiated contractions at either level of PO2 .	manualset1
81586	4	358032	5	NULL	NULL	0	NULL	serotonin 	NonProteinOrNucleicAcidChemical		does not modulate					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	( ii ) The nitric oxide synthase inhibitor N omega-nitro-L-arginine methyl ester ( L-NAME , 100 microM ) did not modulate 5-HT-initiated contractions at either level of PO2 .	manualset1
81587	1	358037	5	NULL	NULL	0	NULL	Placental implantation site	AnatomicalPart		is not related to					labor	BiologicalProcess	duration of			NULL		0	NULL	NULL	NULL	NULL	NULL	( p less than 0.05 ) 4 ) Placental implantation site had no relation with labor duration , fetal weight , placental weight , amount of hemorrhage during labor and cord-coiling .	manualset1
81588	2	358037	5	NULL	NULL	0	NULL	Placental implantation site	AnatomicalPart		is not related to					fetal weight	QuantityOrMeasure				NULL		0	NULL	NULL	NULL	NULL	NULL	( p less than 0.05 ) 4 ) Placental implantation site had no relation with labor duration , fetal weight , placental weight , amount of hemorrhage during labor and cord-coiling .	manualset1
81589	3	358037	5	NULL	NULL	0	NULL	Placental implantation site	AnatomicalPart		is not related to					placental weight	QuantityOrMeasure				NULL		0	NULL	NULL	NULL	NULL	NULL	( p less than 0.05 ) 4 ) Placental implantation site had no relation with labor duration , fetal weight , placental weight , amount of hemorrhage during labor and cord-coiling .	manualset1
81590	5	358037	5	NULL	NULL	0	NULL	Placental implantation site	AnatomicalPart		is not related to					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	( p less than 0.05 ) 4 ) Placental implantation site had no relation with labor duration , fetal weight , placental weight , amount of hemorrhage during labor and cord-coiling .	manualset1
81591	4	358037	5	NULL	NULL	0	NULL	hemorrhage	MedicalFinding		occurs during					labor	BiologicalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	( p less than 0.05 ) 4 ) Placental implantation site had no relation with labor duration , fetal weight , placental weight , amount of hemorrhage during labor and cord-coiling .	manualset1
81592	6	358037	5	NULL	NULL	0	NULL	Placental implantation site	AnatomicalPart		is not related to					cord-coiling	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	( p less than 0.05 ) 4 ) Placental implantation site had no relation with labor duration , fetal weight , placental weight , amount of hemorrhage during labor and cord-coiling .	manualset1
81593	1	358054	5	NULL	NULL	0	NULL	endosome	CellComponent		is regulated to					Golgi pathway	BiologicalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	- arrestins therefore seem to regulate an endosome to Golgi pathway used by multiple cargo proteins .	manualset1
81594	2	358054	5	NULL	NULL	0	NULL	arrestins	Protein		plays a role in					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	- arrestins therefore seem to regulate an endosome to Golgi pathway used by multiple cargo proteins .	manualset1
81595	1	358055	5	NULL	NULL	0	NULL	cell-cell adhesion	BiologicalProcess		is followed by					fusion	BiologicalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	- catenin is a molecular switch that regulates transition of cell-cell adhesion to fusion .	manualset1
81596	2	358055	5	NULL	NULL	0	NULL	catenin	Protein		is a type of					molecular switch	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	- catenin is a molecular switch that regulates transition of cell-cell adhesion to fusion .	manualset1
81597	3	358055	5	NULL	NULL	0	NULL	catenin	Protein		regulate					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	- catenin is a molecular switch that regulates transition of cell-cell adhesion to fusion .	manualset1
81598	1	358057	5	NULL	NULL	0	NULL	immunological phenomena	Process		located in					epidermis	AnatomicalPart	psoriatic 			NULL		0	NULL	NULL	NULL	NULL	NULL	- this alteration in cell membranes results from immunological phenomena located in psoriatic epidermis .	manualset1
81599	2	358057	5	NULL	NULL	0	NULL	statement 1	Process		alters					cell membrane	AnatomicalPart				NULL		0	NULL	NULL	NULL	NULL	NULL	- this alteration in cell membranes results from immunological phenomena located in psoriatic epidermis .	manualset1
81812	1	358065	5	NULL	NULL	0	NULL	Leukotrienes	NonProteinOrNucleicAcidChemical		constitutes					bioactive mediators	NonProteinOrNucleicAcidChemical	class of;;potent			NULL		0	NULL	NULL	NULL	NULL	NULL	1 Leukotrienes constitute a class of potent bioactive mediators known to play a pivotal role in inflammation .	manualset1
81813	2	358065	5	NULL	NULL	0	NULL	statement 1	NonProteinOrNucleicAcidChemical		plays a role in		pivotal			inflammation	BiologicalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	1 Leukotrienes constitute a class of potent bioactive mediators known to play a pivotal role in inflammation .	manualset1
81815	1	358077	5	NULL	NULL	0	NULL	1,7-Azulenequinones	NonProteinOrNucleicAcidChemical		shows					cytotoxicity	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	1,5 - and 1,7-Azulenequinones generally showed higher cytotoxicity , as compared with tropolones and azulene derivatives .	manualset1
81817	2	358077	5	NULL	NULL	0	NULL	1,5-Azulenequinones	NonProteinOrNucleicAcidChemical		shows					cytotoxicity	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	1,5 - and 1,7-Azulenequinones generally showed higher cytotoxicity , as compared with tropolones and azulene derivatives .	manualset1
81818	3	358077	5	NULL	NULL	0	NULL	tropolones	NonProteinOrNucleicAcidChemical		shows					cytotoxicity	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	1,5 - and 1,7-Azulenequinones generally showed higher cytotoxicity , as compared with tropolones and azulene derivatives .	manualset1
81819	4	358077	5	NULL	NULL	0	NULL	azulene derivatives	NonProteinOrNucleicAcidChemical		shows					cytotoxicity	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	1,5 - and 1,7-Azulenequinones generally showed higher cytotoxicity , as compared with tropolones and azulene derivatives .	manualset1
81820	5	358077	5	NULL	NULL	0	NULL	statement 1	Process		is higher in					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	1,5 - and 1,7-Azulenequinones generally showed higher cytotoxicity , as compared with tropolones and azulene derivatives .	manualset1
81821	6	358077	5	NULL	NULL	0	NULL	statement 1	Process		is higher than					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	1,5 - and 1,7-Azulenequinones generally showed higher cytotoxicity , as compared with tropolones and azulene derivatives .	manualset1
81822	7	358077	5	NULL	NULL	0	NULL	statement 2	Process		is higher than					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	1,5 - and 1,7-Azulenequinones generally showed higher cytotoxicity , as compared with tropolones and azulene derivatives .	manualset1
81823	8	358077	5	NULL	NULL	0	NULL	statement 2	Process		is higher than					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	1,5 - and 1,7-Azulenequinones generally showed higher cytotoxicity , as compared with tropolones and azulene derivatives .	manualset1
81824	1	358080	5	NULL	NULL	0	NULL	1-Carboxymethyl-3-hydroxy-2-methyl-4-pyridone	NonProteinOrNucleicAcidChemical		is obtained from					isomaltol	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	1-Carboxymethyl-3-hydroxy-2-methyl-4-pyridone is obtained from isomaltol and glycine .	manualset1
81825	2	358080	5	NULL	NULL	0	NULL	1-Carboxymethyl-3-hydroxy-2-methyl-4-pyridone	NonProteinOrNucleicAcidChemical		is obtained from					glycine	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	1-Carboxymethyl-3-hydroxy-2-methyl-4-pyridone is obtained from isomaltol and glycine .	manualset1
81826	1	358081	5	NULL	NULL	0	NULL	MPTP 	NonProteinOrNucleicAcidChemical		is					1-Methyl-4-phenyl-1 ,2,3,6 - tetrahydropyridine	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	1-Methyl-4-phenyl-1 ,2,3,6 - tetrahydropyridine ( MPTP ) - induced neurotoxicity is the most common experimental model used to investigate the pathogenesis of PD .	manualset1
81827	2	358081	5	NULL	NULL	0	NULL	MPTP 	NonProteinOrNucleicAcidChemical		induce					neurotoxicity	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	1-Methyl-4-phenyl-1 ,2,3,6 - tetrahydropyridine ( MPTP ) - induced neurotoxicity is the most common experimental model used to investigate the pathogenesis of PD .	manualset1
81828	3	358081	5	NULL	NULL	0	NULL	MPTP	NonProteinOrNucleicAcidChemical		is used to 					PD	Disease	investigate;;pathogenesis of			NULL		0	NULL	NULL	NULL	NULL	NULL	1-Methyl-4-phenyl-1 ,2,3,6 - tetrahydropyridine ( MPTP ) - induced neurotoxicity is the most common experimental model used to investigate the pathogenesis of PD .	manualset1
81829	1	358085	5	NULL	NULL	0	NULL	IKCa	NonProteinOrNucleicAcidChemical		is					non-inactivating current	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	10 % of cells ) showed only a non-inactivating current ( IKCa ) which was blocked by 2 mM TEA .	manualset1
81830	2	358085	5	NULL	NULL	0	NULL	IKCa	NonProteinOrNucleicAcidChemical		is blocked by					TEA	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	10 % of cells ) showed only a non-inactivating current ( IKCa ) which was blocked by 2 mM TEA .	manualset1
81831	1	358093	5	NULL	NULL	NULL	NULL	10-23 type deoxyribozymes	Protein		more active than					8-17 type deoxyribozymes	Protein				NULL		NULL	NULL	NULL	NULL	NULL	NULL	10-23 type deoxyribozymes generally appeared more active than 8-17 type and it was possible to predict deoxyribozymes with high cleavage efficiency using scanning array hybridization and computational analysis as guides .	manualset1
81832	1	358100	5	NULL	NULL	0	NULL	11 beta-HSD	Protein		is					11 beta-hydroxysteroid dehydrogenase	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	11 beta-hydroxysteroid dehydrogenase ( 11 beta-HSD ) catalyzes the interconversion of cortisol ( F ) to inactive cortisone ( E ) in man ( corticosterone ( B ) to 11-dehydrocorticosterone ( A ) in rodents ) and plays a crucial role in regulating corticosteroid hormone action .	manualset1
81833	2	358100	5	NULL	NULL	0	NULL	cortisol	Chemical		is interconverted to					cortisone	Chemical				NULL	man	0	NULL	NULL	NULL	NULL	NULL	11 beta-hydroxysteroid dehydrogenase ( 11 beta-HSD ) catalyzes the interconversion of cortisol ( F ) to inactive cortisone ( E ) in man ( corticosterone ( B ) to 11-dehydrocorticosterone ( A ) in rodents ) and plays a crucial role in regulating corticosteroid hormone action .	manualset1
81834	3	358100	5	NULL	NULL	NULL	NULL	corticosterone ( B )	Chemical		is interconverted to					1-dehydrocorticosterone ( A )	Chemical				NULL	rodents	NULL	NULL	NULL	NULL	NULL	NULL	11 beta-hydroxysteroid dehydrogenase ( 11 beta-HSD ) catalyzes the interconversion of cortisol ( F ) to inactive cortisone ( E ) in man ( corticosterone ( B ) to 11-dehydrocorticosterone ( A ) in rodents ) and plays a crucial role in regulating corticosteroid hormone action .	manualset1
81835	4	358100	5	NULL	NULL	0	NULL	11 beta-HSD	Protein		catalyzes					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	11 beta-hydroxysteroid dehydrogenase ( 11 beta-HSD ) catalyzes the interconversion of cortisol ( F ) to inactive cortisone ( E ) in man ( corticosterone ( B ) to 11-dehydrocorticosterone ( A ) in rodents ) and plays a crucial role in regulating corticosteroid hormone action .	manualset1
81836	5	358100	5	NULL	NULL	0	NULL	11 beta-HSD	Protein		catalyzes					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	11 beta-hydroxysteroid dehydrogenase ( 11 beta-HSD ) catalyzes the interconversion of cortisol ( F ) to inactive cortisone ( E ) in man ( corticosterone ( B ) to 11-dehydrocorticosterone ( A ) in rodents ) and plays a crucial role in regulating corticosteroid hormone action .	manualset1
81837	6	358100	5	NULL	NULL	0	NULL	11 beta-HSD	Protein		regulates					corticosteroid hormone 	Chemical	action of			NULL		0	NULL	NULL	NULL	NULL	NULL	11 beta-hydroxysteroid dehydrogenase ( 11 beta-HSD ) catalyzes the interconversion of cortisol ( F ) to inactive cortisone ( E ) in man ( corticosterone ( B ) to 11-dehydrocorticosterone ( A ) in rodents ) and plays a crucial role in regulating corticosteroid hormone action .	manualset1
81838	1	358106	5	NULL	NULL	0	NULL	125I-Antisauvagine-30	PartOfProtein		is a type of					novel and specific high-affinity radioligand	PartOfProtein				NULL		0	NULL	NULL	NULL	NULL	NULL	125I-Antisauvagine-30 : a novel and specific high-affinity radioligand for the characterization of corticotropin-releasing factor type 2 receptors .	manualset1
81839	2	358106	5	NULL	NULL	0	NULL	125I-Antisauvagine-30	PartOfProtein		is used in					corticotropin-releasing factor type 2 receptors	Protein	characterization of			NULL		0	NULL	NULL	NULL	NULL	NULL	125I-Antisauvagine-30 : a novel and specific high-affinity radioligand for the characterization of corticotropin-releasing factor type 2 receptors .	manualset1
81840	1	358107	5	NULL	NULL	0	NULL	125I-BoNT type B	Protein		interacts with					motor nerve terminal	BodyPart				NULL	 in vitro	0	NULL	NULL	NULL	NULL	NULL	125I-BoNT type B , applied in vitro to the murine neuromuscular junction , interacts likewise with the motor nerve terminal except that a lower proportion of internalized radioactivity is seen .	manualset1
81841	2	358107	5	NULL	NULL	0	NULL	statement 1	Process		occurs in					neuromuscular junction	BodyPart	murine			NULL	in vitro	0	NULL	NULL	NULL	NULL	NULL	125I-BoNT type B , applied in vitro to the murine neuromuscular junction , interacts likewise with the motor nerve terminal except that a lower proportion of internalized radioactivity is seen .	manualset1
81842	1	358123	5	NULL	NULL	0	NULL	16S rDNA	NucleicAcidSubstance		is not present in					Setaria equina	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	16S rDNA was not found in the equine filarial nematode Setaria equina , using either polymerase chain reaction ( PCR ) or DNA hybridization .	manualset1
81843	2	358123	5	NULL	NULL	0	NULL	Setaria equina	Organism		is a type of					equine filarial nematode	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	16S rDNA was not found in the equine filarial nematode Setaria equina , using either polymerase chain reaction ( PCR ) or DNA hybridization .	manualset1
81844	1	358140	5	NULL	NULL	NULL	NULL	2 ' ( 3 ' ) - O-L-Aminoacyl derivatives of `` bridged '' adenine ribonucleosides	Chemical		is a substrate for					fibosomal peptidyltransferase	Protein				NULL		NULL	NULL	NULL	NULL	NULL	NULL	2 ' ( 3 ' ) - O-L-Aminoacyl derivatives of `` bridged '' adenine ribonucleosides as substrates for fibosomal peptidyltransferase .	manualset1
81845	1	358145	5	NULL	NULL	0	NULL	 intravascular pressure	BiologicalProcess	elevation of	reduce		significantly			G-actin	GeneOrProtein	cytosolic concentration of			NULL		0	NULL	NULL	NULL	NULL	NULL	2 ) The cytosolic concentration of G-actin is significantly reduced by an elevation in intravascular pressure , demonstrating the dynamic nature of actin within VSM and implying a shift in the F : G equilibrium in favor of F-actin .	manualset1
81846	2	358145	5	NULL	NULL	0	NULL	 F : G equilibrium	BiologicalProcess		shifted					F-actin	GeneOrProtein	in favor of			NULL		0	NULL	NULL	NULL	NULL	NULL	2 ) The cytosolic concentration of G-actin is significantly reduced by an elevation in intravascular pressure , demonstrating the dynamic nature of actin within VSM and implying a shift in the F : G equilibrium in favor of F-actin .	manualset1
81847	3	358145	5	NULL	NULL	0	NULL	statement 1	Process		implies					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	2 ) The cytosolic concentration of G-actin is significantly reduced by an elevation in intravascular pressure , demonstrating the dynamic nature of actin within VSM and implying a shift in the F : G equilibrium in favor of F-actin .	manualset1
81848	4	358145	5	NULL	NULL	0	NULL	actin	GeneOrProtein		is dynamic within					VSM	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	2 ) The cytosolic concentration of G-actin is significantly reduced by an elevation in intravascular pressure , demonstrating the dynamic nature of actin within VSM and implying a shift in the F : G equilibrium in favor of F-actin .	manualset1
81849	5	358145	5	NULL	NULL	0	NULL	statement 1	Process		demonstrates					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	2 ) The cytosolic concentration of G-actin is significantly reduced by an elevation in intravascular pressure , demonstrating the dynamic nature of actin within VSM and implying a shift in the F : G equilibrium in favor of F-actin .	manualset1
81872	1	358154	5	NULL	NULL	0	NULL	Digitoxin	NonProteinOrNucleicAcidChemical		produce					inotropic responses	BiologicalProcess	greatest			NULL		0	NULL	NULL	NULL	NULL	NULL	2 Digitoxin produced the greatest inotropic responses in this series , while the sequence of cleavage products produced progressively smaller responses .	manualset1
81884	1	358160	5	NULL	NULL	0	NULL	2,3-butanediol	NonProteinOrNucleicAcidChemical		produced by					acetogenic bacteria	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	2,3-butanediol production by acetogenic bacteria , an alternative route to chemical synthesis , using industrial waste gas .	manualset1
81885	2	358160	5	NULL	NULL	0	NULL	statement 1	Process		uses					waste gas	NonProteinOrNucleicAcidChemical	industrial			NULL		0	NULL	NULL	NULL	NULL	NULL	2,3-butanediol production by acetogenic bacteria , an alternative route to chemical synthesis , using industrial waste gas .	manualset1
81886	3	358160	5	NULL	NULL	0	NULL	statement 1	Process		is an alternative route to					chemical synthesis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	2,3-butanediol production by acetogenic bacteria , an alternative route to chemical synthesis , using industrial waste gas .	manualset1
81888	1	358161	5	NULL	NULL	0	NULL	2,4-Diamino-5 - ( 5 ' - ( 5-carboxypentyl ) -2 ' - methoxybenzyl ) pyrimidine	Chemical		is more potent than					TMP	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	2,4-Diamino-5 - ( 5 ' - ( 5-carboxypentyl ) -2 ' - methoxybenzyl ) pyrimidine ( 6 ) had a selectivity index of 490 against Tg DHFR and was 320 times more potent than TMP .	manualset1
81107	1	366696	6	NULL	NULL	0	NULL	bisacodyl	Chemical		decreases					ATPase	Protein	activity of			NULL	colonic	0	NULL	NULL	NULL	NULL	NULL	Eighteen hours after its intragastric administration , bisacodyl ( 5.9 mg/kg body wt ) decreased significantly jejunal and colonic ( Na + K ) ATPase activity : 36.4 + / - 1.4 ( SE ) and 28.3 + / - 1.4 , respectively , as compared to 42.1 + / - 1.6 and 37.0 + / - 2.9 mumol/mg protein/hr in saline-treated rats .	manualset1
81129	1	366706	6	NULL	NULL	NULL	NULL	interleukin 1-receptor	GP	elaboration of 	is not attenuated by					glucocorticoids	NonProteinOrNucleicAcidChemical				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Elaboration of interleukin 1-receptor antagonist is not attenuated by glucocorticoids after endotoxemia .	manualset1
81131	2	366706	6	NULL	NULL	0	NULL	statement 1	Process		occurs after					endotoxemia	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Elaboration of interleukin 1-receptor antagonist is not attenuated by glucocorticoids after endotoxemia .	manualset1
81132	1	366707	6	NULL	NULL	0	NULL	Elastic fibers	AnatomicalPart		are fragmented in					arterial walls	BodyPart	pulmonary			NULL		0	NULL	NULL	NULL	NULL	NULL	Elastic fibers in E18 .5 Lox ( - / - ) lungs were markedly less intensely stained and more disperse than in the wild type , especially in the mesenchyme surrounding the distal airways , bronchioles , bronchi , and trachea , and were fragmented in pulmonary arterial walls .	manualset1
81133	1	366708	6	NULL	NULL	0	NULL	Elastin peptides	Protein		are present in					serum	Protein	human			NULL		0	NULL	NULL	NULL	NULL	NULL	Elastin peptides derived from the degradation are present in human sera .	manualset1
81134	2	366708	6	NULL	NULL	0	NULL	Elastin peptides	Protein		is derived from					degradation	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Elastin peptides derived from the degradation are present in human sera .	manualset1
81135	1	366709	6	NULL	NULL	0	NULL	Elastosis	Disease		deposits					elastin	Protein	large amounts of 			NULL		0	NULL	NULL	NULL	NULL	NULL	Elastosis , the deposition of large amounts of elastin , is characteristic of the desmoplastic reaction to human breast carcinoma .	manualset1
81136	2	366709	6	NULL	NULL	NULL	NULL	Elastosis	Disease		is characteristic of 					Breast Carcinoma	Disease	human;; desmoplastic reaction to 			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Elastosis , the deposition of large amounts of elastin , is characteristic of the desmoplastic reaction to human breast carcinoma .	manualset1
81141	1	366720	6	NULL	NULL	0	NULL	S3	SmallMolecule	electrical stimulation of	results in					sphincter component	CellComponent	visible contraction of;; striated;; muscular;; anal			NULL		0	NULL	NULL	NULL	NULL	NULL	Electrical stimulation of S3 and S4 results in visible contraction of the different striated muscular anal sphincter components and in an increase of anal canal closure pressure .	manualset1
81142	2	366720	6	NULL	NULL	0	NULL	S4	SmallMolecule	electrical stimulation of	results in					sphincter component	CellComponent	visible contraction of;; striated;; muscular;; anal			NULL		0	NULL	NULL	NULL	NULL	NULL	Electrical stimulation of S3 and S4 results in visible contraction of the different striated muscular anal sphincter components and in an increase of anal canal closure pressure .	manualset1
81146	1	366723	6	NULL	NULL	0	NULL	dorsal raphe 	BodyPart	stimulation of 	inhibits					DA neurons	CellComponent	firing rate of 			NULL		0	NULL	NULL	NULL	NULL	NULL	Electrical stimulation of the dorsal raphe selectively inhibited the firing rate of slowly firing ( less than 4 spikes/sec ) DA neurons .	manualset1
81160	1	366734	6	NULL	NULL	NULL	NULL	electrolyte	Chemical	leakage of	is indicative of					membrane	CellComponent	perturbation of 			NULL	C. herbarum	NULL	NULL	NULL	NULL	NULL	NULL	Electrolyte leakage , indicative of membrane perturbation , was evident in both C. herbarum and B. cinerea exposed to 4-octyl cyclopentenone .	manualset1
81162	2	366734	6	NULL	NULL	0	NULL	electrolyte	Chemical	leakage of	is indicative of					membrane	CellComponent	perturbation of 			NULL	B. cinerea	0	NULL	NULL	NULL	NULL	NULL	Electrolyte leakage , indicative of membrane perturbation , was evident in both C. herbarum and B. cinerea exposed to 4-octyl cyclopentenone .	manualset1
81163	3	366734	6	NULL	NULL	0	NULL	statement 1	Process		occurs after					4-octyl cyclopentenone	NonProteinOrNucleicAcidChemical	exposure to			NULL		0	NULL	NULL	NULL	NULL	NULL	Electrolyte leakage , indicative of membrane perturbation , was evident in both C. herbarum and B. cinerea exposed to 4-octyl cyclopentenone .	manualset1
81164	4	366734	6	NULL	NULL	0	NULL	statement 2	Process		occurs after					4-octyl cyclopentenone	NonProteinOrNucleicAcidChemical	exposure to			NULL		0	NULL	NULL	NULL	NULL	NULL	Electrolyte leakage , indicative of membrane perturbation , was evident in both C. herbarum and B. cinerea exposed to 4-octyl cyclopentenone .	manualset1
81168	1	366738	6	NULL	NULL	0	NULL	orbicularis oris muscles	BodyPart	upper	produces					speech	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Electromyographic analysis of the upper and lower orbicularis oris muscles in the production of speech .	manualset1
81170	2	366738	6	NULL	NULL	0	NULL	orbicularis oris muscles	BodyPart	lower	produces					speech	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Electromyographic analysis of the upper and lower orbicularis oris muscles in the production of speech .	manualset1
81176	1	366739	6	NULL	NULL	0	NULL	depressor labii inferior muscle	BodyPart	right	does not have					voluntary activity	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Electromyographic examination showed absent voluntary activity of the right depressor labii inferior muscle .	manualset1
81179	1	366746	6	NULL	NULL	0	NULL	epithelial autograft	MedicalProcedure	cultured;; healed	lacks					dermal attachments	AnatomicalPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Electron microscopic examination of a biopsy specimen of the healed cultured epithelial autograft ( 80 days after placement ) revealed a lack of dermal attachments of the anchoring fibrils .	manualset1
81181	2	366746	6	NULL	NULL	0	NULL	statement 1	Process		occurs in					fibrils	CellComponent	anchoring			NULL		0	NULL	NULL	NULL	NULL	NULL	Electron microscopic examination of a biopsy specimen of the healed cultured epithelial autograft ( 80 days after placement ) revealed a lack of dermal attachments of the anchoring fibrils .	manualset1
81197	1	366747	6	NULL	NULL	0	NULL	microtubular deposits	CellComponent		are present in					glomeruli	CellComponent	subendothelial space of			NULL		0	NULL	NULL	NULL	NULL	NULL	Electron microscopic examination revealed microtubular and fibrillary deposits with diameters of 80-100 and 9-16 nm , respectively , in the subendothelial space of the glomeruli .	manualset1
81198	1	366754	6	NULL	NULL	0	NULL	microfibrils	CellComponent	exposed appearance of	decreases					elastin	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	Electron microscopy of dermal elastic fibers showed a decreased amount of elastin with an exposed appearance of microfibrils .	manualset1
81199	1	366758	6	NULL	NULL	0	NULL	DMPO	Chemical		is					5 , 5-dimethyl-1-pyrroline-N-oxide	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Electron spin resonance spectroscopy studies using 5 , 5-dimethyl-1-pyrroline-N-oxide ( DMPO ) as a spin trap indicate a complete inhibition of hydroxyl radical formation via the iron-catalyzed Fenton reaction at molar phytic acid/iron ratios ) 5 .	manualset1
81200	2	366758	6	NULL	NULL	0	NULL	DMPO	Chemical		inhibits					hydroxyl radical	Chemical	formation of 			NULL		0	NULL	NULL	NULL	NULL	NULL	Electron spin resonance spectroscopy studies using 5 , 5-dimethyl-1-pyrroline-N-oxide ( DMPO ) as a spin trap indicate a complete inhibition of hydroxyl radical formation via the iron-catalyzed Fenton reaction at molar phytic acid/iron ratios ) 5 .	manualset1
81203	1	366764	6	NULL	NULL	0	NULL	ouabain	Chemical		induces					ventricular dysrhythmias	Disease				NULL	rabbit	0	NULL	NULL	NULL	NULL	NULL	Electrophysiologic effects of potassium canrenoate on ouabain-induced ventricular dysrhythmias in rabbits .	manualset1
81333	1	366768	6	NULL	NULL	0	NULL	ultrafine fibers	AnatomicalPart	electrospun	increases					dissolution	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Electrospun ultrafine fibers increased the dissolution more effectively , owing to the formed solid solution and huge surface .	manualset1
81210	1	366773	6	NULL	NULL	0	NULL	antiganglioside antibodies 	Protein	elevated	is secondary to					axons	CellComponent	damage to			NULL		0	NULL	NULL	NULL	NULL	NULL	Elevated antiganglioside antibodies may be secondary to axonal damage or may be a cause of axonal damage and accumulating disability in progressive MS. In either case , they may serve as a marker of axonal damage in MS.	manualset1
81211	2	366773	6	NULL	NULL	0	NULL	antiganglioside antibodies 	Protein		may cause					MS	Disease	progressive;; disability in 			NULL		0	NULL	NULL	NULL	NULL	NULL	Elevated antiganglioside antibodies may be secondary to axonal damage or may be a cause of axonal damage and accumulating disability in progressive MS. In either case , they may serve as a marker of axonal damage in MS.	manualset1
81212	1	366775	6	NULL	NULL	0	NULL	SHBG-cholesterol	NonProteinOrNucleicAcidChemical	concentration of 	increases					luteal phase	BiologicalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Elevated concentrations of SHBG and HDL-cholesterol and a suppression of LDL-cholesterol were found during the luteal compared to the follicular phase and these findings were interpreted as an estrogenic influence .	manualset1
81213	2	366775	6	NULL	NULL	0	NULL	HDL-cholesterol	NonProteinOrNucleicAcidChemical	concentration of 	increases during					luteal phase	BiologicalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Elevated concentrations of SHBG and HDL-cholesterol and a suppression of LDL-cholesterol were found during the luteal compared to the follicular phase and these findings were interpreted as an estrogenic influence .	manualset1
81214	1	366776	6	NULL	NULL	0	NULL	corticosterone	NonProteinOrNucleicAcidChemical	elevated	affects					body size					NULL		0	NULL	NULL	NULL	NULL	NULL	Elevated corticosterone levels during embryonic development affected body size , growth rates , and sex ratios of the resultant offspring , but the direction and magnitude of these effects differed between the species .	manualset1
81215	2	366776	6	NULL	NULL	0	NULL	corticosterone	NonProteinOrNucleicAcidChemical	elevated	affects					growth rate	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Elevated corticosterone levels during embryonic development affected body size , growth rates , and sex ratios of the resultant offspring , but the direction and magnitude of these effects differed between the species .	manualset1
81216	3	366776	6	NULL	NULL	0	NULL	corticosterone	NonProteinOrNucleicAcidChemical	elevated	affects					sex ratios					NULL		0	NULL	NULL	NULL	NULL	NULL	Elevated corticosterone levels during embryonic development affected body size , growth rates , and sex ratios of the resultant offspring , but the direction and magnitude of these effects differed between the species .	manualset1
81336	1	366777	6	NULL	NULL	NULL	NULL	T-bet	GeneOrProtein	elevated expression of 	increases					Th1 cell 	cell	differentiation of			NULL	T-EP67-vaccinated mice	NULL	NULL	NULL	NULL	NULL	NULL	Elevated expression of T-bet and RORc transcription factors in T-EP67-vaccinated mice indicated the promotion of Th1 and Th17 cell differentiation .	manualset1
81342	2	366777	6	NULL	NULL	NULL	NULL	RORc	GeneOrProtein	elevated expression of 	increases					Th17 cell	cell	differentiation of			NULL	T-EP67-vaccinated mice	NULL	NULL	NULL	NULL	NULL	NULL	Elevated expression of T-bet and RORc transcription factors in T-EP67-vaccinated mice indicated the promotion of Th1 and Th17 cell differentiation .	manualset1
81358	1	366778	6	NULL	NULL	0	NULL	testosterone	Protein	maternal;; elevated levels of 	results in					2D:4D 	Protein	lower			NULL		0	NULL	NULL	NULL	NULL	NULL	Elevated levels of maternal testosterone resulted in lower 2D :4 D ratios and an elongated 4D on the left and right forepaws in both males and females .	manualset1
81362	1	366779	6	NULL	NULL	0	NULL	testosterone	Protein	elevated levels of 	results in					2D:4D 	Protein	lower			NULL		0	NULL	NULL	NULL	NULL	NULL	Elevated proline aminopeptidase activity has been identified as a reliable marker enzyme for bacterial vaginosis .	manualset1
81582	1	366780	6	NULL	NULL	0	NULL	serum IgE	Protein	elevated	reflects					immune regulation	BiologicalProcess	defective			NULL		0	NULL	NULL	NULL	NULL	NULL	Elevated serum IgE probably reflects defective immune regulation .	manualset1
79102	1	376994	7	NULL	NULL	NULL	NULL	Nevirapine nanosuspensions	NonProteinOrNucleicAcidChemical		target					HIV reservoir	organism				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nevirapine nanosuspensions for HIV reservoir targeting .	manualset1
79633	1	377001	7	NULL	NULL	0	NULL	Mycobacterium avium complex 	Organism	agents active against	selected										NULL		0	NULL	NULL	NULL	NULL	NULL	New agents active against Mycobacterium avium complex selected by molecular topology : a virtual screening method .	manualset1
79634	1	377002	7	NULL	NULL	0	NULL	curcumin	NonProteinOrNucleicAcidChemical	New analogs of	required for					therapeutics	MedicalProcedureOrDevice				NULL		0	NULL	NULL	NULL	NULL	NULL	New analogs of curcumin with improved properties are needed to meet therapeutic requirements .	manualset1
79635	1	377004	7	NULL	NULL	0	NULL	anemia	MedicalFinding		occur during					preconception	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	New chapters are added concerning anemia during preconception and the puerperium .	manualset1
79636	2	377004	7	NULL	NULL	0	NULL	anemia	MedicalFinding		occur during					puerperium	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	New chapters are added concerning anemia during preconception and the puerperium .	manualset1
79637	1	377011	7	NULL	NULL	0	NULL	cisplatin	NonProteinOrNucleicAcidChemical		shows					extracellular resistance mechanism	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	New extracellular resistance mechanism for cisplatin .	manualset1
79661	1	377014	7	NULL	NULL	0	NULL	archaeosomes	NonProteinOrNucleicAcidChemical		belongs to					liposomes	NonProteinOrNucleicAcidChemical	new generation of			NULL		0	NULL	NULL	NULL	NULL	NULL	New generation of liposomes called archaeosomes based on natural or synthetic archaeal lipids as innovative formulations for drug delivery .	manualset1
79662	2	377014	7	NULL	NULL	NULL	NULL	archaeosomes	NonProteinOrNucleicAcidChemical		based on					natural archaeal lipids	NonProteinOrNucleicAcidChemical				NULL		NULL	NULL	NULL	NULL	NULL	NULL	New generation of liposomes called archaeosomes based on natural or synthetic archaeal lipids as innovative formulations for drug delivery .	manualset1
79663	3	377014	7	NULL	NULL	0	NULL	archaeosomes	NonProteinOrNucleicAcidChemical		based on					synthetic archaeal lipids	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	New generation of liposomes called archaeosomes based on natural or synthetic archaeal lipids as innovative formulations for drug delivery .	manualset1
79664	4	377014	7	NULL	NULL	0	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	New generation of liposomes called archaeosomes based on natural or synthetic archaeal lipids as innovative formulations for drug delivery .	manualset1
79665	5	377014	7	NULL	NULL	0	NULL	archaeosomes	NonProteinOrNucleicAcidChemical		formulations for		innovative			drug delivery	MedicalProcedureOrDevice				NULL		0	NULL	NULL	NULL	NULL	NULL	New generation of liposomes called archaeosomes based on natural or synthetic archaeal lipids as innovative formulations for drug delivery .	manualset1
79666	1	377015	7	NULL	NULL	0	NULL	TPO	Protein		is involved in					ET	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	New insights are emerging into the role of the megakaryocytopoiesis regulator thrombopoietin ( TPO ) and its receptor , c-Mpl , in ET and related disorders , but TPO-Mpl dynamics appear to be complex .	manualset1
79667	2	377015	7	NULL	NULL	0	NULL	c-Mpl	GeneOrProtein		is involved in					ET	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	New insights are emerging into the role of the megakaryocytopoiesis regulator thrombopoietin ( TPO ) and its receptor , c-Mpl , in ET and related disorders , but TPO-Mpl dynamics appear to be complex .	manualset1
79668	3	377015	7	NULL	NULL	0	NULL	TPO	Protein		is					 thrombopoietin	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	New insights are emerging into the role of the megakaryocytopoiesis regulator thrombopoietin ( TPO ) and its receptor , c-Mpl , in ET and related disorders , but TPO-Mpl dynamics appear to be complex .	manualset1
79669	4	377015	7	NULL	NULL	0	NULL	TPO	Protein		is a type of					megakaryocytopoiesis regulator	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	New insights are emerging into the role of the megakaryocytopoiesis regulator thrombopoietin ( TPO ) and its receptor , c-Mpl , in ET and related disorders , but TPO-Mpl dynamics appear to be complex .	manualset1
79688	1	377022	7	NULL	NULL	0	NULL	psychotropic drugs	NonProteinOrNucleicAcidChemical		cure					plasmids	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	NULL	NULL	New mechanism of plasmid curing by psychotropic drugs .	manualset1
79689	1	377025	7	NULL	NULL	0	NULL	New oscillometric method	MedicalProcedureOrDevice		measures		indirectly			systolic arterial pressure	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	New oscillometric method for indirect measurement of systolic and mean arterial pressure in the human finger .	manualset1
79690	2	377025	7	NULL	NULL	0	NULL	New oscillometric method	MedicalProcedureOrDevice		measures		indirectly			mean arterial pressure	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	New oscillometric method for indirect measurement of systolic and mean arterial pressure in the human finger .	manualset1
79691	3	377025	7	NULL	NULL	0	NULL	statement 1	Process		occur in					 finger	BodyPart	human			NULL		0	NULL	NULL	NULL	NULL	NULL	New oscillometric method for indirect measurement of systolic and mean arterial pressure in the human finger .	manualset1
79692	4	377025	7	NULL	NULL	0	NULL	statement 2	Process		occur in					finger	BodyPart	human			NULL		0	NULL	NULL	NULL	NULL	NULL	New oscillometric method for indirect measurement of systolic and mean arterial pressure in the human finger .	manualset1
79739	1	377027	7	NULL	NULL	NULL	NULL	receptor-linked phospholipase D	Protein	coupling of	occur in					neutrophils	Cell	primed			NULL		NULL	NULL	NULL	NULL	NULL	NULL	New pathways of phagocyte activation : the coupling of receptor-linked phospholipase D and the role of tyrosine kinase in primed neutrophils .	manualset1
79740	2	377027	7	NULL	NULL	0	NULL	tyrosine kinase	Protein		participate in					phagocyte	Cell	activation of			NULL		0	NULL	NULL	NULL	NULL	NULL	New pathways of phagocyte activation : the coupling of receptor-linked phospholipase D and the role of tyrosine kinase in primed neutrophils .	manualset1
79741	3	377027	7	NULL	NULL	NULL	NULL	statement 1	Process		participate in					phagocyte	Cell	activation of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	New pathways of phagocyte activation : the coupling of receptor-linked phospholipase D and the role of tyrosine kinase in primed neutrophils .	manualset1
79742	4	377027	7	NULL	NULL	0	NULL	statement 1	Process		occur in					neutrophils	Cell	primed			NULL		0	NULL	NULL	NULL	NULL	NULL	New pathways of phagocyte activation : the coupling of receptor-linked phospholipase D and the role of tyrosine kinase in primed neutrophils .	manualset1
79743	1	377028	7	NULL	NULL	0	NULL	 mucAB	GeneOrProtein		associated with					new phenotype	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	New phenotypes associated with mucAB : alteration of a MucA sequence homologous to the LexA cleavage site .	manualset1
79744	2	377030	7	NULL	NULL	NULL	NULL	Fas2 gene	Gene	site-directed mutagenesis of;;synthetic	designed to					statement 1	Process	delineate the individual contributions of 			NULL		NULL	NULL	NULL	NULL	NULL	NULL	New probes , designed to delineate the individual contributions of the fasciculin residues to the complex formation and conformation , were generated by site-directed mutagenesis of a synthetic Fas2 gene .	manualset1
79745	1	377030	7	NULL	NULL	0	NULL	fasciculin residues	AminoAcid		forms					complex	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	New probes , designed to delineate the individual contributions of the fasciculin residues to the complex formation and conformation , were generated by site-directed mutagenesis of a synthetic Fas2 gene .	manualset1
79746	1	377033	7	NULL	NULL	0	NULL	rifampin	NonProteinOrNucleicAcidChemical	resistance to	detected in					Mycobacterium tuberculosis	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	New rapid phenotypic assays for the detection of rifampin resistance in Mycobacterium tuberculosis have recently been described , but most of these require liquid cultures , which reduces the utility of many tests in terms of turnaround times .	manualset1
79747	1	377039	7	NULL	NULL	0	NULL	New therapeutic approaches	MedicalProcedureOrDevice		based on					antimicrotubules agents	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	New therapeutic approaches are now based on antimicrotubules agents but it is difficult to evaluate their efficacity .	manualset1
79748	1	377040	7	NULL	NULL	0	NULL	New vascular graft	BodyPart		simplifies					aortic valve reimplantation technique	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	New vascular graft for simplification of the aortic valve reimplantation technique .	manualset1
79749	1	377041	7	NULL	NULL	0	NULL	New vesicular ampicillin-loaded delivery systems 	MedicalProcedureOrDevice		used for					topical application	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	New vesicular ampicillin-loaded delivery systems for topical application : characterization , in vitro permeation experiments and antimicrobial activity .	manualset1
79750	1	377044	7	NULL	NULL	NULL	NULL	Newer fluoroquinolones	NonProteinOrNucleicAcidChemical		activity against		increased;;in vitro			anaerobes	Organism				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Newer fluoroquinolones with increased in vitro activity against anaerobes are under development and include levofloxacin , clinafloxacin , sparfloxacin , trovafloxacin , grepafloxacin , and DU-6859a .	manualset1
79751	2	377044	7	NULL	NULL	0	NULL	levofloxacin	NonProteinOrNucleicAcidChemical		is a type of					Newer fluoroquinolones	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Newer fluoroquinolones with increased in vitro activity against anaerobes are under development and include levofloxacin , clinafloxacin , sparfloxacin , trovafloxacin , grepafloxacin , and DU-6859a .	manualset1
79752	3	377044	7	NULL	NULL	0	NULL	 clinafloxacin	NonProteinOrNucleicAcidChemical		is a type of					Newer fluoroquinolones	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Newer fluoroquinolones with increased in vitro activity against anaerobes are under development and include levofloxacin , clinafloxacin , sparfloxacin , trovafloxacin , grepafloxacin , and DU-6859a .	manualset1
79753	4	377044	7	NULL	NULL	0	NULL	sparfloxacin	NonProteinOrNucleicAcidChemical		is a type of					Newer fluoroquinolones	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Newer fluoroquinolones with increased in vitro activity against anaerobes are under development and include levofloxacin , clinafloxacin , sparfloxacin , trovafloxacin , grepafloxacin , and DU-6859a .	manualset1
79754	5	377044	7	NULL	NULL	0	NULL	trovafloxacin	NonProteinOrNucleicAcidChemical		is a type of					Newer fluoroquinolones	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Newer fluoroquinolones with increased in vitro activity against anaerobes are under development and include levofloxacin , clinafloxacin , sparfloxacin , trovafloxacin , grepafloxacin , and DU-6859a .	manualset1
79755	6	377044	7	NULL	NULL	0	NULL	grepafloxacin	NonProteinOrNucleicAcidChemical		is a type of					Newer fluoroquinolones	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Newer fluoroquinolones with increased in vitro activity against anaerobes are under development and include levofloxacin , clinafloxacin , sparfloxacin , trovafloxacin , grepafloxacin , and DU-6859a .	manualset1
79756	7	377044	7	NULL	NULL	0	NULL	DU-6859a	NonProteinOrNucleicAcidChemical		is a type of					Newer fluoroquinolones	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Newer fluoroquinolones with increased in vitro activity against anaerobes are under development and include levofloxacin , clinafloxacin , sparfloxacin , trovafloxacin , grepafloxacin , and DU-6859a .	manualset1
79761	1	377045	7	NULL	NULL	NULL	NULL	pancreatic inflammatory disease	Disease	complications of 	include					 pseudocysts	MedicalFinding	percutaneous drainage of 			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Newer management strategies for these complications of pancreatic inflammatory disease are discussed , including percutaneous drainage of pseudocysts and the use of octreotide in the management of pancreatic ascites and pancreatic fistulas .	manualset1
79762	2	377045	7	NULL	NULL	NULL	NULL	octreotide	NonProteinOrNucleicAcidChemical		used in the					pancreatic ascites 	MedicalFinding	management of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Newer management strategies for these complications of pancreatic inflammatory disease are discussed , including percutaneous drainage of pseudocysts and the use of octreotide in the management of pancreatic ascites and pancreatic fistulas .	manualset1
79763	3	377045	7	NULL	NULL	0	NULL	octreotide	NonProteinOrNucleicAcidChemical		used in the					pancreatic fistulas	MedicalFinding	management of			NULL		0	NULL	NULL	NULL	NULL	NULL	Newer management strategies for these complications of pancreatic inflammatory disease are discussed , including percutaneous drainage of pseudocysts and the use of octreotide in the management of pancreatic ascites and pancreatic fistulas .	manualset1
79765	1	377047	7	NULL	NULL	0	NULL	L-3 ,4 - dihydroxyphenylalanine	NonProteinOrNucleicAcidChemical		converted to					DA	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Next , AtT-20 neuroendocrine cells were transfected with wild-type and mutated TH genes because these cells were earlier shown to be capable of fully converting L-3 ,4 - dihydroxyphenylalanine into DA , whereby the catalytic activity of TH would be expected to be inhibited by the end product DA accumulating in the cells .	manualset1
79766	2	377047	7	NULL	NULL	NULL	NULL	AtT-20 neuroendocrine cells	Cell		transfected with					TH genes	Gene	wildtype			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Next , AtT-20 neuroendocrine cells were transfected with wild-type and mutated TH genes because these cells were earlier shown to be capable of fully converting L-3 ,4 - dihydroxyphenylalanine into DA , whereby the catalytic activity of TH would be expected to be inhibited by the end product DA accumulating in the cells .	manualset1
79767	3	377047	7	NULL	NULL	NULL	NULL	AtT-20 neuroendocrine cells 	Cell		transfected with					TH genes	Gene	mutated			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Next , AtT-20 neuroendocrine cells were transfected with wild-type and mutated TH genes because these cells were earlier shown to be capable of fully converting L-3 ,4 - dihydroxyphenylalanine into DA , whereby the catalytic activity of TH would be expected to be inhibited by the end product DA accumulating in the cells .	manualset1
79768	4	377047	7	NULL	NULL	NULL	NULL	statement 1	Process		occur in					statement 2	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Next , AtT-20 neuroendocrine cells were transfected with wild-type and mutated TH genes because these cells were earlier shown to be capable of fully converting L-3 ,4 - dihydroxyphenylalanine into DA , whereby the catalytic activity of TH would be expected to be inhibited by the end product DA accumulating in the cells .	manualset1
79769	5	377047	7	NULL	NULL	0	NULL	statement 1	Process		occur in					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Next , AtT-20 neuroendocrine cells were transfected with wild-type and mutated TH genes because these cells were earlier shown to be capable of fully converting L-3 ,4 - dihydroxyphenylalanine into DA , whereby the catalytic activity of TH would be expected to be inhibited by the end product DA accumulating in the cells .	manualset1
79770	6	377047	7	NULL	NULL	NULL	NULL	DA	NonProteinOrNucleicAcidChemical		accumulate in					AtT-20 neuroendocrine cells 	Cell				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Next , AtT-20 neuroendocrine cells were transfected with wild-type and mutated TH genes because these cells were earlier shown to be capable of fully converting L-3 ,4 - dihydroxyphenylalanine into DA , whereby the catalytic activity of TH would be expected to be inhibited by the end product DA accumulating in the cells .	manualset1
79771	7	377047	7	NULL	NULL	0	NULL	statement 6	Process		inhibit		may			TH	GeneOrProtein	catalytic activity of			NULL		0	NULL	NULL	NULL	NULL	NULL	Next , AtT-20 neuroendocrine cells were transfected with wild-type and mutated TH genes because these cells were earlier shown to be capable of fully converting L-3 ,4 - dihydroxyphenylalanine into DA , whereby the catalytic activity of TH would be expected to be inhibited by the end product DA accumulating in the cells .	manualset1
79772	8	377047	7	NULL	NULL	0	NULL	statement 2	Process		occur along with					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Next , AtT-20 neuroendocrine cells were transfected with wild-type and mutated TH genes because these cells were earlier shown to be capable of fully converting L-3 ,4 - dihydroxyphenylalanine into DA , whereby the catalytic activity of TH would be expected to be inhibited by the end product DA accumulating in the cells .	manualset1
79773	1	377048	7	NULL	NULL	NULL	NULL	VEGFR2 + cells	Cell	FACS-sorted	express					SMC-specific marker	GeneOrProtein				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Next , FACS-sorted VEGFR2 + cells expressed highest and lowest levels of SMC - and fibroblast-specific markers , respectively , at days 7-14 after retinoic acid ( RA ) as compared with VEGFR2 + / PDGFR + cells .	manualset1
79774	2	377048	7	NULL	NULL	NULL	NULL	VEGFR2 + cells	Cell	FACS-sorted	express					fibroblast-specific marker	GeneOrProtein				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Next , FACS-sorted VEGFR2 + cells expressed highest and lowest levels of SMC - and fibroblast-specific markers , respectively , at days 7-14 after retinoic acid ( RA ) as compared with VEGFR2 + / PDGFR + cells .	manualset1
79775	3	377048	7	NULL	NULL	0	NULL	VEGFR2 + / PDGFR + cells	Cell		express					SMC-specific marker	GeneOrProtein				NULL		0	NULL	NULL	NULL	NULL	NULL	Next , FACS-sorted VEGFR2 + cells expressed highest and lowest levels of SMC - and fibroblast-specific markers , respectively , at days 7-14 after retinoic acid ( RA ) as compared with VEGFR2 + / PDGFR + cells .	manualset1
79776	4	377048	7	NULL	NULL	0	NULL	VEGFR2 + / PDGFR + cells	Cell		express					fibroblast-specific marker	GeneOrProtein				NULL		0	NULL	NULL	NULL	NULL	NULL	Next , FACS-sorted VEGFR2 + cells expressed highest and lowest levels of SMC - and fibroblast-specific markers , respectively , at days 7-14 after retinoic acid ( RA ) as compared with VEGFR2 + / PDGFR + cells .	manualset1
79777	5	377048	7	NULL	NULL	0	NULL	statement 1	Process		is higher than					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Next , FACS-sorted VEGFR2 + cells expressed highest and lowest levels of SMC - and fibroblast-specific markers , respectively , at days 7-14 after retinoic acid ( RA ) as compared with VEGFR2 + / PDGFR + cells .	manualset1
79778	6	377048	7	NULL	NULL	0	NULL	statement 2	Process		is higher than					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Next , FACS-sorted VEGFR2 + cells expressed highest and lowest levels of SMC - and fibroblast-specific markers , respectively , at days 7-14 after retinoic acid ( RA ) as compared with VEGFR2 + / PDGFR + cells .	manualset1
79781	1	377052	7	NULL	NULL	0	NULL	pWEE1B	GeneOrProtein		localize in					nucleus	CellComponent				NULL		0	NULL	NULL	NULL	NULL	NULL	Next , the localization of pWEE1B was examined by immunohistochemistry , and exclusive nuclear localization was revealed in the fully grown oocytes .	manualset1
79782	2	377052	7	NULL	NULL	0	NULL	statement 1	Process		occur in					oocytes	Cell	fully grown			NULL		0	NULL	NULL	NULL	NULL	NULL	Next , the localization of pWEE1B was examined by immunohistochemistry , and exclusive nuclear localization was revealed in the fully grown oocytes .	manualset1
79783	1	377055	7	NULL	NULL	0	NULL	UFH	NonProteinOrNucleicAcidChemical		is a type of		well-established			 intravenous therapy	MedicalProcedure	concomitant			NULL		0	NULL	NULL	NULL	NULL	NULL	Next to antiplatelet therapy , unfractionated heparin ( UFH ) is a well-established concomitant intravenous therapy during PCI .	manualset1
79784	2	377055	7	NULL	NULL	0	NULL	statement 1	Process		occur during					PCI	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Next to antiplatelet therapy , unfractionated heparin ( UFH ) is a well-established concomitant intravenous therapy during PCI .	manualset1
79785	3	377055	7	NULL	NULL	0	NULL	UFH	NonProteinOrNucleicAcidChemical		is 					unfractionated heparin	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Next to antiplatelet therapy , unfractionated heparin ( UFH ) is a well-established concomitant intravenous therapy during PCI .	manualset1
79786	4	377055	7	NULL	NULL	0	NULL	statement 1	Process		is used					antiplatelet therapy	MedicalProcedure	next to			NULL		0	NULL	NULL	NULL	NULL	NULL	Next to antiplatelet therapy , unfractionated heparin ( UFH ) is a well-established concomitant intravenous therapy during PCI .	manualset1
79787	1	377056	7	NULL	NULL	0	NULL	Nicergoline	NonProteinOrNucleicAcidChemical		enhances					glutamate 	AminoAcid	re-uptake of			NULL		0	NULL	NULL	NULL	NULL	NULL	Nicergoline enhances glutamate re-uptake and protects against brain damage in rat global brain ischemia .	manualset1
79788	2	377056	7	NULL	NULL	0	NULL	statement 1	Process		protects against					brain 	BodyPart	damage of			NULL		0	NULL	NULL	NULL	NULL	NULL	Nicergoline enhances glutamate re-uptake and protects against brain damage in rat global brain ischemia .	manualset1
79789	3	377056	7	NULL	NULL	NULL	NULL	statement 2	Process		occur in					global brain ischemia	Disease	rat			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nicergoline enhances glutamate re-uptake and protects against brain damage in rat global brain ischemia .	manualset1
79791	1	377057	7	NULL	NULL	NULL	NULL	Nickel	Chemical		catalyze					vinyl epoxides	NonProteinOrNucleicAcidChemical	borylative ring opening of 			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nickel-catalyzed borylative ring opening of vinyl epoxides and aziridines .	manualset1
79792	2	377057	7	NULL	NULL	NULL	NULL	Nickel	Chemical		catalyze					aziridines	NonProteinOrNucleicAcidChemical	borylative ring opening of 			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nickel-catalyzed borylative ring opening of vinyl epoxides and aziridines .	manualset1
79793	1	377058	7	NULL	NULL	NULL	NULL	Nicotinamide	NonProteinOrNucleicAcidChemical		decreases					nitric oxide	NonProteinOrNucleicAcidChemical	production of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nicotinamide decreases nitric oxide production and partially protects human pancreatic islets against the suppressive effects of combinations of cytokines .	manualset1
79794	2	377058	7	NULL	NULL	0	NULL	statement 1	Process		protects		partially			pancreatic islets	BodyPart	human			NULL		0	NULL	NULL	NULL	NULL	NULL	Nicotinamide decreases nitric oxide production and partially protects human pancreatic islets against the suppressive effects of combinations of cytokines .	manualset1
79795	3	377058	7	NULL	NULL	0	NULL	statement 2	Process		against					cytokines	NonProteinOrNucleicAcidChemical	 suppressive effects of combinations of			NULL		0	NULL	NULL	NULL	NULL	NULL	Nicotinamide decreases nitric oxide production and partially protects human pancreatic islets against the suppressive effects of combinations of cytokines .	manualset1
79796	1	377059	7	NULL	NULL	NULL	NULL	Nicotine	NonProteinOrNucleicAcidChemical		interacts with					opioid 	NonProteinOrNucleicAcidChemical				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nicotine 's opioid and anti-opioid interactions : proposed role in smoking behavior .	manualset1
79797	2	377059	7	NULL	NULL	NULL	NULL	Nicotine	NonProteinOrNucleicAcidChemical		interacts with					anti-opioid	NonProteinOrNucleicAcidChemical				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nicotine 's opioid and anti-opioid interactions : proposed role in smoking behavior .	manualset1
79798	1	377062	7	NULL	NULL	NULL	NULL	array CGH	MedicalProcedureOrDevice		used to					chromosome 18	Chromosome	 illustrate the aberrations of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nine cases of aberrations involving chromosome 18 are used to illustrate the use and clinical potential of array CGH .	manualset1
79799	1	377064	7	NULL	NULL	0	NULL	 moss species 	Organism		shows					antibacterial activity	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nine moss species showed antibacterial activity against Gram ( + ) bacteria , in particular H. splendens and its ethyl acetate fractions showed stronger activity .	manualset1
79800	2	377064	7	NULL	NULL	0	NULL	statement 1	Process		against					 H. splendens	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Nine moss species showed antibacterial activity against Gram ( + ) bacteria , in particular H. splendens and its ethyl acetate fractions showed stronger activity .	manualset1
79801	3	377064	7	NULL	NULL	0	NULL	 H. splendens	Organism		is a type of					Gram ( + ) bacteria	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Nine moss species showed antibacterial activity against Gram ( + ) bacteria , in particular H. splendens and its ethyl acetate fractions showed stronger activity .	manualset1
79802	1	377067	7	NULL	NULL	NULL	NULL	hypothyroidism	Disease		occur due to					thyroid ectopia	Disease				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nine patients suffering from hypothyroidism due to thyroid ectopia or hypogenesis , with a large sella turcica , were examined at adolescence or during adult life .	manualset1
79803	2	377067	7	NULL	NULL	NULL	NULL	hypothyroidism	Disease		occur due to					large sella turcica	BodyPart	hypogenesis with			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nine patients suffering from hypothyroidism due to thyroid ectopia or hypogenesis , with a large sella turcica , were examined at adolescence or during adult life .	manualset1
79804	1	377070	7	NULL	NULL	0	NULL	ATIII	Protein		used in the					 venous thrombosis	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	Nine subjects with acquired ATIII deficiency also received ATIII treatment for venous or arterial thrombosis or disseminated intravascular coagulation , all with low plasma ATIII levels .	manualset1
79805	2	377070	7	NULL	NULL	0	NULL	ATIII	Protein		used in the					arterial thrombosis	MedicalFinding	treatment of			NULL		0	NULL	NULL	NULL	NULL	NULL	Nine subjects with acquired ATIII deficiency also received ATIII treatment for venous or arterial thrombosis or disseminated intravascular coagulation , all with low plasma ATIII levels .	manualset1
79806	3	377070	7	NULL	NULL	NULL	NULL	ATIII	Protein		used in the					disseminated intravascular coagulation	BiologicalProcess	treatment of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nine subjects with acquired ATIII deficiency also received ATIII treatment for venous or arterial thrombosis or disseminated intravascular coagulation , all with low plasma ATIII levels .	manualset1
79807	4	377070	7	NULL	NULL	0	NULL	venous thrombosis	MedicalFinding		occur due to					ATIII	Protein	deficiency of			NULL		0	NULL	NULL	NULL	NULL	NULL	Nine subjects with acquired ATIII deficiency also received ATIII treatment for venous or arterial thrombosis or disseminated intravascular coagulation , all with low plasma ATIII levels .	manualset1
79808	5	377070	7	NULL	NULL	0	NULL	arterial thrombosis	MedicalFinding		occur due to					ATIII	Protein	deficiency of			NULL		0	NULL	NULL	NULL	NULL	NULL	Nine subjects with acquired ATIII deficiency also received ATIII treatment for venous or arterial thrombosis or disseminated intravascular coagulation , all with low plasma ATIII levels .	manualset1
79809	6	377070	7	NULL	NULL	0	NULL	disseminated intravascular coagulation	BiologicalProcess		occur due to					ATIII	Protein	deficiency of			NULL		0	NULL	NULL	NULL	NULL	NULL	Nine subjects with acquired ATIII deficiency also received ATIII treatment for venous or arterial thrombosis or disseminated intravascular coagulation , all with low plasma ATIII levels .	manualset1
79810	1	377074	7	NULL	NULL	NULL	NULL	PAG 	BodyPart	stimulation of	relieves					back pain	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nineteen patients with both leg and back pain received electrodes in the PAG and the somatosensory regions ; whereas back pain was relieved by PAG stimulation , dysesthetic leg pain was controlled more effectively by somatosensory region stimulation .	manualset1
79811	2	377074	7	NULL	NULL	0	NULL	somatosensory region	BodyPart	stimulation of	controls		effectively			dysesthetic leg pain	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Nineteen patients with both leg and back pain received electrodes in the PAG and the somatosensory regions ; whereas back pain was relieved by PAG stimulation , dysesthetic leg pain was controlled more effectively by somatosensory region stimulation .	manualset1
79812	1	377077	7	NULL	NULL	0	NULL	dichloromethane	Chemical	crude extracts with	used in the					Yemeni ethnomedicine	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety crude extracts , including dichloromethane , methanol and aqueous extracts from 30 medicinal plants used in the Yemeni ethnomedicine to treat common infections , were screened in vitro for antimicrobial activities against three Gram-positive bacteria and two Gram-negative bacteria , Candida maltosa and five opportunistic human fungal pathogens ( two yeasts , three hyphomycetes ) .	manualset1
79813	2	377077	7	NULL	NULL	0	NULL	methanol	Chemical	crude extracts with	used in the					Yemeni ethnomedicine	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety crude extracts , including dichloromethane , methanol and aqueous extracts from 30 medicinal plants used in the Yemeni ethnomedicine to treat common infections , were screened in vitro for antimicrobial activities against three Gram-positive bacteria and two Gram-negative bacteria , Candida maltosa and five opportunistic human fungal pathogens ( two yeasts , three hyphomycetes ) .	manualset1
79814	1	377078	7	NULL	NULL	0	NULL	male F344 rats	Organism	tumors induced in	harbor					mutations	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety percent ( 18 of 20 ) of the tumors induced in male F344 rats harbored mutations , which were detected in three of four adenomas ( 75 % ) and 15 of 16 adenocarcinomas ( 94 % ) .	manualset1
79816	1	377089	7	NULL	NULL	0	NULL	NitR	GeneOrProtein		regulator of					hmgA	GeneOrProtein	S. meliloti;;expression of			NULL		0	NULL	NULL	NULL	NULL	NULL	NitR was found to be a regulator of S. meliloti hmgA expression under nitrogen deprivation conditions , suggesting the presence of a ntr-independent nitrogen deprivation regulatory system .	manualset1
79817	2	377089	7	NULL	NULL	0	NULL	statement 1	Process		under					nitrogen	Chemical	deprivation condition of			NULL		0	NULL	NULL	NULL	NULL	NULL	NitR was found to be a regulator of S. meliloti hmgA expression under nitrogen deprivation conditions , suggesting the presence of a ntr-independent nitrogen deprivation regulatory system .	manualset1
79818	3	377089	7	NULL	NULL	0	NULL	statement 1	Process		suggest					ntr-independent nitrogen deprivation regulatory system	BiologicalProcess	presence of			NULL		0	NULL	NULL	NULL	NULL	NULL	NitR was found to be a regulator of S. meliloti hmgA expression under nitrogen deprivation conditions , suggesting the presence of a ntr-independent nitrogen deprivation regulatory system .	manualset1
79819	1	377090	7	NULL	NULL	0	NULL	Nitrates	Chemical		likely to be					active substances	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Nitrates are very likely to be active substances on Holter recorded angina but no controlled studies have been performed to really demonstrate it .	manualset1
79820	2	377090	7	NULL	NULL	0	NULL	statement 1	Process		occur on					Holter recorded angina	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Nitrates are very likely to be active substances on Holter recorded angina but no controlled studies have been performed to really demonstrate it .	manualset1
79821	1	377091	7	NULL	NULL	NULL	NULL	NO	NonProteinOrNucleicAcidChemical		play a role in					sensory activity	BiologicalProcess				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nitric oxide ( NO ) in the spinal cord plays a role in sensory and autonomic activity .	manualset1
79822	2	377091	7	NULL	NULL	NULL	NULL	NO	NonProteinOrNucleicAcidChemical		play a role in					autonomic activity	BiologicalProcess				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nitric oxide ( NO ) in the spinal cord plays a role in sensory and autonomic activity .	manualset1
79823	3	377091	7	NULL	NULL	0	NULL	statement 1	Process		occur in the					spinal cord	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide ( NO ) in the spinal cord plays a role in sensory and autonomic activity .	manualset1
79824	4	377091	7	NULL	NULL	NULL	NULL	statement 2	Process		occur in the					spinal cord	BodyPart				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nitric oxide ( NO ) in the spinal cord plays a role in sensory and autonomic activity .	manualset1
79825	5	377091	7	NULL	NULL	0	NULL	NO	Chemical		is					Nitric oxide	Chemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide ( NO ) in the spinal cord plays a role in sensory and autonomic activity .	manualset1
79848	1	377092	7	NULL	NULL	NULL	NULL	NO	NonProteinOrNucleicAcidChemical	production of	enhanced in					active ulcerative colitis	Disease				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nitric oxide ( NO ) production , as detectable by indirect and direct methods , as well as the expression of inducible nitric oxide synthase ( iNOS ) in the intestinal mucosa appear to be enhanced in active ulcerative colitis and , when in excess , to play a proinflammatory role in the disease .	manualset1
79850	2	377092	7	NULL	NULL	0	NULL	iNOS	Protein	expression of	enhanced in					active ulcerative colitis	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide ( NO ) production , as detectable by indirect and direct methods , as well as the expression of inducible nitric oxide synthase ( iNOS ) in the intestinal mucosa appear to be enhanced in active ulcerative colitis and , when in excess , to play a proinflammatory role in the disease .	manualset1
79851	3	377092	7	NULL	NULL	0	NULL	statement 1	Process		occur in					intestinal mucosa	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide ( NO ) production , as detectable by indirect and direct methods , as well as the expression of inducible nitric oxide synthase ( iNOS ) in the intestinal mucosa appear to be enhanced in active ulcerative colitis and , when in excess , to play a proinflammatory role in the disease .	manualset1
79852	4	377092	7	NULL	NULL	0	NULL	statement 2	Process		occur in					intestinal mucosa	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide ( NO ) production , as detectable by indirect and direct methods , as well as the expression of inducible nitric oxide synthase ( iNOS ) in the intestinal mucosa appear to be enhanced in active ulcerative colitis and , when in excess , to play a proinflammatory role in the disease .	manualset1
79854	5	377092	7	NULL	NULL	NULL	NULL	NO	NonProteinOrNucleicAcidChemical	excess of	proinflammatory role in					active ulcerative colitis	Disease				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nitric oxide ( NO ) production , as detectable by indirect and direct methods , as well as the expression of inducible nitric oxide synthase ( iNOS ) in the intestinal mucosa appear to be enhanced in active ulcerative colitis and , when in excess , to play a proinflammatory role in the disease .	manualset1
79860	6	377092	7	NULL	NULL	0	NULL	iNOS	Protein	excess of	proinflammatory role in					active ulcerative colitis	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide ( NO ) production , as detectable by indirect and direct methods , as well as the expression of inducible nitric oxide synthase ( iNOS ) in the intestinal mucosa appear to be enhanced in active ulcerative colitis and , when in excess , to play a proinflammatory role in the disease .	manualset1
79861	7	377092	7	NULL	NULL	0	NULL	NO	NonProteinOrNucleicAcidChemical		is					Nitric oxide	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide ( NO ) production , as detectable by indirect and direct methods , as well as the expression of inducible nitric oxide synthase ( iNOS ) in the intestinal mucosa appear to be enhanced in active ulcerative colitis and , when in excess , to play a proinflammatory role in the disease .	manualset1
79862	8	377092	7	NULL	NULL	0	NULL	iNOS	Protein		is					inducible nitric oxide synthase 	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide ( NO ) production , as detectable by indirect and direct methods , as well as the expression of inducible nitric oxide synthase ( iNOS ) in the intestinal mucosa appear to be enhanced in active ulcerative colitis and , when in excess , to play a proinflammatory role in the disease .	manualset1
79898	1	377095	7	NULL	NULL	0	NULL	NO donors 	NonProteinOrNucleicAcidChemical		produce		exogenously			Nitric oxide	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide produced exogenously by the addition of NO donors was able to delay or inhibit apoptosis induced by a combination of tumor necrosis factor alpha and actinomycin D and to suppress the activity of caspase 3 .	manualset1
79899	2	377095	7	NULL	NULL	0	NULL	tumor necrosis factor alpha	Protein		induce					apoptosis	MolecularProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide produced exogenously by the addition of NO donors was able to delay or inhibit apoptosis induced by a combination of tumor necrosis factor alpha and actinomycin D and to suppress the activity of caspase 3 .	manualset1
79900	3	377095	7	NULL	NULL	0	NULL	actinomycin D	NonProteinOrNucleicAcidChemical		induce					apoptosis	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide produced exogenously by the addition of NO donors was able to delay or inhibit apoptosis induced by a combination of tumor necrosis factor alpha and actinomycin D and to suppress the activity of caspase 3 .	manualset1
79901	4	377095	7	NULL	NULL	0	NULL	statement 2	Process		in combination with					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide produced exogenously by the addition of NO donors was able to delay or inhibit apoptosis induced by a combination of tumor necrosis factor alpha and actinomycin D and to suppress the activity of caspase 3 .	manualset1
79902	5	377095	7	NULL	NULL	0	NULL	Nitric oxide	NonProteinOrNucleicAcidChemical		delay					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide produced exogenously by the addition of NO donors was able to delay or inhibit apoptosis induced by a combination of tumor necrosis factor alpha and actinomycin D and to suppress the activity of caspase 3 .	manualset1
79903	6	377095	7	NULL	NULL	0	NULL	Nitric oxide	NonProteinOrNucleicAcidChemical		inhibit					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide produced exogenously by the addition of NO donors was able to delay or inhibit apoptosis induced by a combination of tumor necrosis factor alpha and actinomycin D and to suppress the activity of caspase 3 .	manualset1
79904	7	377095	7	NULL	NULL	0	NULL	statement 5	Process		is an alternative to					statement 6	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide produced exogenously by the addition of NO donors was able to delay or inhibit apoptosis induced by a combination of tumor necrosis factor alpha and actinomycin D and to suppress the activity of caspase 3 .	manualset1
79905	8	377095	7	NULL	NULL	0	NULL	Nitric oxide	NonProteinOrNucleicAcidChemical		suppress					caspase 3	Protein	activity of			NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide produced exogenously by the addition of NO donors was able to delay or inhibit apoptosis induced by a combination of tumor necrosis factor alpha and actinomycin D and to suppress the activity of caspase 3 .	manualset1
79906	1	377096	7	NULL	NULL	0	NULL	Nitric oxide	NonProteinOrNucleicAcidChemical	release of	reduce					psoriasis	Disease	incidence of cutaneous infections in			NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide release accounts for the reduced incidence of cutaneous infections in psoriasis .	manualset1
79907	1	377097	7	NULL	NULL	0	NULL	aminoguanidine	NonProteinOrNucleicAcidChemical	pentacycloundecane conjugates of	inhibit					Nitric oxide synthase	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide synthase inhibition by pentacycloundecane conjugates of aminoguanidine and tryptamine .	manualset1
79908	2	377097	7	NULL	NULL	NULL	NULL	tryptamine	NonProteinOrNucleicAcidChemical	pentacycloundecane conjugates of	inhibit					Nitric oxide synthase	Protein				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nitric oxide synthase inhibition by pentacycloundecane conjugates of aminoguanidine and tryptamine .	manualset1
79910	1	377100	7	NULL	NULL	0	NULL	risedronate	NonProteinOrNucleicAcidChemical		inhibit					farnesyl diphosphate synthase	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	Nitrogen-containing bisphosphonate drugs such as risedronate act by inhibiting farnesyl diphosphate synthase , thereby disrupting protein prenylation in osteoclasts .	manualset1
79911	2	377100	7	NULL	NULL	NULL	NULL	statement 1	Process		disrupt					protein prenylation	MolecularProcess				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nitrogen-containing bisphosphonate drugs such as risedronate act by inhibiting farnesyl diphosphate synthase , thereby disrupting protein prenylation in osteoclasts .	manualset1
79912	3	377100	7	NULL	NULL	0	NULL	statement 1	Process		occur in					osteoclasts	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Nitrogen-containing bisphosphonate drugs such as risedronate act by inhibiting farnesyl diphosphate synthase , thereby disrupting protein prenylation in osteoclasts .	manualset1
79913	4	377100	7	NULL	NULL	0	NULL	risedronate	NonProteinOrNucleicAcidChemical		is a type of					Nitrogen-containing bisphosphonate drugs	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Nitrogen-containing bisphosphonate drugs such as risedronate act by inhibiting farnesyl diphosphate synthase , thereby disrupting protein prenylation in osteoclasts .	manualset1
79917	1	377101	7	NULL	NULL	NULL	NULL	Nitroglycerin	NonProteinOrNucleicAcidChemical		decrease					t-PA	Protein	thrombolytic effect of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nitroglycerin given with tissue-type plasminogen activator ( t-PA ) has been shown to decrease the thrombolytic effect of t-PA in animal models of coronary artery thrombosis .	manualset1
79918	2	377101	7	NULL	NULL	0	NULL	statement 1	Process		occur in					coronary artery thrombosis	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Nitroglycerin given with tissue-type plasminogen activator ( t-PA ) has been shown to decrease the thrombolytic effect of t-PA in animal models of coronary artery thrombosis .	manualset1
79919	3	377101	7	NULL	NULL	0	NULL	statement 1	Process		along with					t-PA	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	Nitroglycerin given with tissue-type plasminogen activator ( t-PA ) has been shown to decrease the thrombolytic effect of t-PA in animal models of coronary artery thrombosis .	manualset1
79920	4	377101	7	NULL	NULL	0	NULL	t-PA	Protein		is					tissue-type plasminogen activator	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	Nitroglycerin given with tissue-type plasminogen activator ( t-PA ) has been shown to decrease the thrombolytic effect of t-PA in animal models of coronary artery thrombosis .	manualset1
79933	1	377103	7	NULL	NULL	0	NULL	Nitromethane	NonProteinOrNucleicAcidChemical		is used as					methyl 	Chemical	suitable photolytic precursor of 			NULL		0	NULL	NULL	NULL	NULL	NULL	Nitromethane was identified as a particularly suitable photolytic precursor of methyl for studies by photoionization and threshold photoelectron spectroscopy .	manualset1
79939	2	377103	7	NULL	NULL	0	NULL	statement 1	Process		is used in					photoionization studies	ResearchActivity				NULL		0	NULL	NULL	NULL	NULL	NULL	Nitromethane was identified as a particularly suitable photolytic precursor of methyl for studies by photoionization and threshold photoelectron spectroscopy .	manualset1
79940	3	377103	7	NULL	NULL	0	NULL	statement 1	Process		is used in					threshold photoelectron spectroscopy	ResearchActivity				NULL		0	NULL	NULL	NULL	NULL	NULL	Nitromethane was identified as a particularly suitable photolytic precursor of methyl for studies by photoionization and threshold photoelectron spectroscopy .	manualset1
79942	1	377104	7	NULL	NULL	0	NULL	 peroxynitrite	NonProteinOrNucleicAcidChemical		mediate					damage	BiologicalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Nitrotyrosine detection in plasma and tissues may be a useful method to demonstrate peroxynitrite-mediated damage .	manualset1
79944	2	377104	7	NULL	NULL	NULL	NULL	Nitrotyrosine 	NonProteinOrNucleicAcidChemical	detection of	demonstrate					statement 1	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nitrotyrosine detection in plasma and tissues may be a useful method to demonstrate peroxynitrite-mediated damage .	manualset1
79945	3	377104	7	NULL	NULL	0	NULL	statement 1	Process		occur in					plasma	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Nitrotyrosine detection in plasma and tissues may be a useful method to demonstrate peroxynitrite-mediated damage .	manualset1
79946	4	377104	7	NULL	NULL	0	NULL	statement 1	Process		occur in					tissues	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Nitrotyrosine detection in plasma and tissues may be a useful method to demonstrate peroxynitrite-mediated damage .	manualset1
79947	1	377105	7	NULL	NULL	0	NULL	Nitrous oxide	NonProteinOrNucleicAcidChemical		becomes					dentists	PersonGroup	vice of			NULL		0	NULL	NULL	NULL	NULL	NULL	Nitrous oxide becomes the vice of dentists .	manualset1
79948	1	377106	7	NULL	NULL	0	NULL	Nm23	GeneOrProtein		expressed in					tissue specimens	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Nm23 was found to be expressed in all the tissue specimens .	manualset1
79949	1	377109	7	NULL	NULL	0	NULL	Gs protein 	Protein		not detected in					CT1-producing cultures	LaboratoryExperimentalFactor				NULL		0	NULL	NULL	NULL	NULL	NULL	No Gs protein could be detected in the CT1-producing cultures .	manualset1
79988	1	377118	7	NULL	NULL	0	NULL	IL-6	Protein	levels of	not associated with					knee extensor muscle 	BodyPart	strength of			NULL		0	NULL	NULL	NULL	NULL	NULL	No association was found between IL-6 levels and knee extensor muscle ( r = 0.087 , P = 0.306 ) or flexor ( r = -0.011 , P = 0.894 ) strength .	manualset1
80011	1	377126	7	NULL	NULL	0	NULL	 light heteropaenia	Disease		detected in					chicks	Organism	CIAV-vaccinated			NULL		0	NULL	NULL	NULL	NULL	NULL	No clinical signs were observed but light heteropaenia was detected in CIAV-vaccinated chicks .	manualset1
80024	1	377128	7	NULL	NULL	0	NULL	anti-LPS antibody	Protein	regulation of	different with					anti-Ipa antibody	Protein	regulation of			NULL		0	NULL	NULL	NULL	NULL	NULL	No close correlations between the anti-LPS and anti-Ipa antibody responses were observed indicating that they may be differently regulated .	manualset1
80025	1	377134	7	NULL	NULL	NULL	NULL	deformability	BiologicalProcess	decrease in	not correlated with					extracorporeal circulation procedure	MedicalProcedure	duration of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	No correlation was found between decrease in deformability and duration of the extracorporeal circulation procedure .	manualset1
80260	1	377144	7	NULL	NULL	NULL	NULL	PPMS	Disease	 QoL of	does not differ with					progressive MS	Disease	QoL of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	No difference in QoL was found between patients with PPMS and those with secondary progressive MS. The Italian FAMS questionnaire is a valid measure to assess the QoL concerns of patients with MS. FAMS is also easy to administer and is well accepted by patients .	manualset1
80261	1	377145	7	NULL	NULL	0	NULL	sLepR mRNA	Gene	 level of brain;;fish fed reduced	does not differ with					sLepR mRNA	Gene	level of brain;;fish full feeded			NULL		0	NULL	NULL	NULL	NULL	NULL	No difference in brain sLepR mRNA levels was observed between fish fed reduced and full feeding regimes .	manualset1
80262	1	377159	7	NULL	NULL	NULL	NULL	clinical toxicity	MedicalFinding		not found in					plasma aluminium	Chemical	patients with maintained			NULL		NULL	NULL	NULL	NULL	NULL	NULL	No evidence of clinical toxicity was found in patients in whom the plasma aluminum was maintained up to 5 mumol/l .	manualset1
80263	1	377160	7	NULL	NULL	0	NULL	renal parenchymal pathologies	MedicalFinding	evidence of	is not implicated in					systemic hypertension 	MedicalFinding	etiology of			NULL		0	NULL	NULL	NULL	NULL	NULL	No evidence of renal parenchymal pathologies implicated in the etiology of systemic hypertension was observed , therefore , these animals would seem to be suitable models for human essential hypertension .	manualset1
80264	1	377163	7	NULL	NULL	0	NULL	NirBD	GeneOrProtein		required for		exclusively			assimilatory nitrite 	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	No functional redundancy between the genes was observed and we demonstrate that NirBD is exclusively required for assimilatory nitrite ( it does not detoxify nitrite ) and SirA exclusively for assimilatory sulfite reduction .	manualset1
80265	2	377163	7	NULL	NULL	0	NULL	NirBD	GeneOrProtein		does not detoxify					nitrite	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	No functional redundancy between the genes was observed and we demonstrate that NirBD is exclusively required for assimilatory nitrite ( it does not detoxify nitrite ) and SirA exclusively for assimilatory sulfite reduction .	manualset1
80266	3	377163	7	NULL	NULL	0	NULL	SirA	GeneOrProtein		reduce		exclusively			assimilatory sulfite	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	No functional redundancy between the genes was observed and we demonstrate that NirBD is exclusively required for assimilatory nitrite ( it does not detoxify nitrite ) and SirA exclusively for assimilatory sulfite reduction .	manualset1
80277	1	377175	7	NULL	NULL	0	NULL	primary tumor	MedicalFinding	morphology of	not different from					metastatic tumor	MedicalFinding	morphology of			NULL		0	NULL	NULL	NULL	NULL	NULL	No morphological differences could be observed between the primary and the metastatic tumors .	manualset1
80278	1	377180	7	NULL	NULL	NULL	NULL	thoracotomy	MedicalProcedureOrDevice	 technique of	does not reduce					chronic postthoracotomy pain	MedicalFinding	incidence of 			NULL		NULL	NULL	NULL	NULL	NULL	NULL	No one technique of thoracotomy has been shown to reduce the incidence of chronic postthoracotomy pain .	manualset1
80279	1	377185	7	NULL	NULL	0	NULL	 pathological tracer uptake	MedicalProcedureOrDevice		is not seen					gastric NHL	Disease	in patient with low-grade			NULL		0	NULL	NULL	NULL	NULL	NULL	No pathological tracer uptake was seen in the patient with low-grade gastric NHL of the MALT type .	manualset1
80280	2	377185	7	NULL	NULL	0	NULL	gastric NHL	Disease		is of					MALT type	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	No pathological tracer uptake was seen in the patient with low-grade gastric NHL of the MALT type .	manualset1
80307	1	377186	7	NULL	NULL	0	NULL	CHT	MedicalProcedure		does not cause					gastric perforation	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	No patient experienced gastric perforation or bleeding during CHT .	manualset1
80308	2	377186	7	NULL	NULL	0	NULL	CHT	MedicalProcedure		does not cause					bleeding	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	No patient experienced gastric perforation or bleeding during CHT .	manualset1
80309	1	377211	7	NULL	NULL	NULL	NULL	thiamine 	NonProteinOrNucleicAcidChemical	early stages of deficiency of	does not alter		significantly			M1 muscarinic binding sites	GeneOrProtein	densities of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	No significant alterations in densities of M1 , M2 or total muscarinic binding sites were observed in any brain structure evaluated at either early or late stages of thiamine deficiency .	manualset1
80310	2	377211	7	NULL	NULL	0	NULL	thiamine 	NonProteinOrNucleicAcidChemical	early stages of deficiency of	does not alter		significantly			M2 muscarinic binding sites	GeneOrProtein	densities of			NULL		0	NULL	NULL	NULL	NULL	NULL	No significant alterations in densities of M1 , M2 or total muscarinic binding sites were observed in any brain structure evaluated at either early or late stages of thiamine deficiency .	manualset1
80311	3	377211	7	NULL	NULL	NULL	NULL	thiamine 	NonProteinOrNucleicAcidChemical	early stages of deficiency of	does not alter		significantly			total muscarinic binding sites	GeneOrProtein	densities of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	No significant alterations in densities of M1 , M2 or total muscarinic binding sites were observed in any brain structure evaluated at either early or late stages of thiamine deficiency .	manualset1
80312	4	377211	7	NULL	NULL	0	NULL	thiamine 	NonProteinOrNucleicAcidChemical	late stages of deficiency of	does not alter		significantly			M1 muscarinic binding sites	GeneOrProtein	densities of			NULL		0	NULL	NULL	NULL	NULL	NULL	No significant alterations in densities of M1 , M2 or total muscarinic binding sites were observed in any brain structure evaluated at either early or late stages of thiamine deficiency .	manualset1
80313	5	377211	7	NULL	NULL	0	NULL	thiamine 	NonProteinOrNucleicAcidChemical	late stages of deficiency of	does not alter		significantly			M2 muscarinic binding sites	GeneOrProtein	densities of			NULL		0	NULL	NULL	NULL	NULL	NULL	No significant alterations in densities of M1 , M2 or total muscarinic binding sites were observed in any brain structure evaluated at either early or late stages of thiamine deficiency .	manualset1
80314	6	377211	7	NULL	NULL	0	NULL	thiamine 	NonProteinOrNucleicAcidChemical	late stages of deficiency of	does not alter		significantly			total muscarinic binding sites	GeneOrProtein	densities of			NULL		0	NULL	NULL	NULL	NULL	NULL	No significant alterations in densities of M1 , M2 or total muscarinic binding sites were observed in any brain structure evaluated at either early or late stages of thiamine deficiency .	manualset1
80315	7	377211	7	NULL	NULL	0	NULL	statement 1	Process		occur in					brain	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	No significant alterations in densities of M1 , M2 or total muscarinic binding sites were observed in any brain structure evaluated at either early or late stages of thiamine deficiency .	manualset1
80316	8	377211	7	NULL	NULL	0	NULL	statement 2	Process		occur in					brain	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	No significant alterations in densities of M1 , M2 or total muscarinic binding sites were observed in any brain structure evaluated at either early or late stages of thiamine deficiency .	manualset1
80317	9	377211	7	NULL	NULL	0	NULL	statement 3	Process		occur in					brain	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	No significant alterations in densities of M1 , M2 or total muscarinic binding sites were observed in any brain structure evaluated at either early or late stages of thiamine deficiency .	manualset1
80318	10	377211	7	NULL	NULL	0	NULL	statement 4	Process		occur in					brain	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	No significant alterations in densities of M1 , M2 or total muscarinic binding sites were observed in any brain structure evaluated at either early or late stages of thiamine deficiency .	manualset1
80319	11	377211	7	NULL	NULL	0	NULL	statement 5	Process		occur in					brain	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	No significant alterations in densities of M1 , M2 or total muscarinic binding sites were observed in any brain structure evaluated at either early or late stages of thiamine deficiency .	manualset1
80320	12	377211	7	NULL	NULL	0	NULL	statement 6	Process		occur in					brain	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	No significant alterations in densities of M1 , M2 or total muscarinic binding sites were observed in any brain structure evaluated at either early or late stages of thiamine deficiency .	manualset1
80321	13	377211	7	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	No significant alterations in densities of M1 , M2 or total muscarinic binding sites were observed in any brain structure evaluated at either early or late stages of thiamine deficiency .	manualset1
80322	14	377211	7	NULL	NULL	0	NULL	statement 2	Process		is an alternative to					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	No significant alterations in densities of M1 , M2 or total muscarinic binding sites were observed in any brain structure evaluated at either early or late stages of thiamine deficiency .	manualset1
80323	15	377211	7	NULL	NULL	0	NULL	statement 3	Process		is an alternative to					statement 6	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	No significant alterations in densities of M1 , M2 or total muscarinic binding sites were observed in any brain structure evaluated at either early or late stages of thiamine deficiency .	manualset1
80324	1	377212	7	NULL	NULL	0	NULL	MMP-9	Protein	expression of	not associated with					herniation grade	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	No significant association was found between MMP-9 expression and herniation grade in patients who were 30-60 years or over 60 years of age .	manualset1
80325	1	377213	7	NULL	NULL	0	NULL	maternal smoking	Process		not associated with		significantly			IgE 	Protein	cord plasma levels of			NULL		0	NULL	NULL	NULL	NULL	NULL	No significant association was observed between maternal smoking and cord plasma IgE levels .	manualset1
80326	1	377216	7	NULL	NULL	0	NULL	Pkcd	Protein		substrate for					caspase 3	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	No significant cleavage of protein kinase C delta ( Pkcd ) in vivo , which is a substrate for caspase 3 , was detected , and intact Pkcd was retained in both cell lines for at least 72 h after irradiation .	manualset1
80327	2	377216	7	NULL	NULL	0	NULL	Pkcd	Protein		is					protein kinase C delta	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	No significant cleavage of protein kinase C delta ( Pkcd ) in vivo , which is a substrate for caspase 3 , was detected , and intact Pkcd was retained in both cell lines for at least 72 h after irradiation .	manualset1
80328	1	377220	7	NULL	NULL	0	NULL	RA1	GeneOrProtein		not different from					RA2	GeneOrProtein				NULL		0	NULL	NULL	NULL	NULL	NULL	No significant difference was observed between RA1 and RA2 .	manualset1
80329	1	377222	7	NULL	NULL	0	NULL	IgG antibody	Protein	levels of;;atopic recruits	does not differ with		significantly			IgG antibody	Protein	levels of;;non-atopic recruits			NULL		0	NULL	NULL	NULL	NULL	NULL	No significant difference was observed in IgG antibody levels to pneumococcal polysaccharides between atopic and non-atopic recruits , whereas seropositivity to T. gondii was found to be less frequent among the atopic recruits ( odds ratio , 0.37 ; 95 % CI , 0.17-0 .81 ; P = 0.01 ) .	manualset1
80330	2	377222	7	NULL	NULL	0	NULL	IgG antibody	Protein		in response to					pneumococcal polysaccharides	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	No significant difference was observed in IgG antibody levels to pneumococcal polysaccharides between atopic and non-atopic recruits , whereas seropositivity to T. gondii was found to be less frequent among the atopic recruits ( odds ratio , 0.37 ; 95 % CI , 0.17-0 .81 ; P = 0.01 ) .	manualset1
80331	3	377222	7	NULL	NULL	0	NULL	T. gondii	Organism	seropositivity to	less frequent among					atopic recruits	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	No significant difference was observed in IgG antibody levels to pneumococcal polysaccharides between atopic and non-atopic recruits , whereas seropositivity to T. gondii was found to be less frequent among the atopic recruits ( odds ratio , 0.37 ; 95 % CI , 0.17-0 .81 ; P = 0.01 ) .	manualset1
80332	1	377229	7	NULL	NULL	0	NULL	2-DG	NonProteinOrNucleicAcidChemical		substrate for					hexokinase	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences were observed in the Km for hexokinase with 2-DG as the substrate in the glioma and normal brain tissue .	manualset1
80333	2	377229	7	NULL	NULL	0	NULL	statement 1	Process		occur in					glioma	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences were observed in the Km for hexokinase with 2-DG as the substrate in the glioma and normal brain tissue .	manualset1
80334	3	377229	7	NULL	NULL	0	NULL	statement 1	Process		occur in					normal brain tissue	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences were observed in the Km for hexokinase with 2-DG as the substrate in the glioma and normal brain tissue .	manualset1
80335	1	377231	7	NULL	NULL	0	NULL	XbaI genotype	Gene		does not effect		significantly			BMD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	No significant effect of the XbaI genotype on BMD was found at any site .	manualset1
80336	1	377237	7	NULL	NULL	0	NULL	spontaneous bleedings	MedicalFinding		does not occur at					birth	BiologicalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	No spontaneous bleedings usually occur at birth in severe type 3 VWD .	manualset1
80337	2	377237	7	NULL	NULL	0	NULL	statement 1	Process		occur in					type 3 VWD	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	No spontaneous bleedings usually occur at birth in severe type 3 VWD .	manualset1
80427	1	377242	7	NULL	NULL	0	NULL	gastrin	Protein		does not stimulate					guanylate cyclase activity	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	No stimulation of guanylate cyclase activity by gastrin was detected in the dispersed gastric corporal mucosal cells .	manualset1
80428	2	377242	7	NULL	NULL	0	NULL	statement 1	Process		occur in					gastric corporal mucosal cells	Cell	dispersed			NULL		0	NULL	NULL	NULL	NULL	NULL	No stimulation of guanylate cyclase activity by gastrin was detected in the dispersed gastric corporal mucosal cells .	manualset1
80429	1	377251	7	NULL	NULL	0	NULL	bcl-1	Gene		involved in					translocations	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	No translocations involving bcl-2 and the immunoglobulin heavy chain gene were identified ; two cases had translocations involving the bcl-1 and the immunoglobulin heavy chain genes .	manualset1
80430	2	377251	7	NULL	NULL	0	NULL	immunoglobulin heavy chain genes	Gene		involved in					translocations	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	No translocations involving bcl-2 and the immunoglobulin heavy chain gene were identified ; two cases had translocations involving the bcl-1 and the immunoglobulin heavy chain genes .	manualset1
80433	1	377258	7	NULL	NULL	0	NULL	Nocardia brain abscess	MedicalFinding		mimick					necrotic tumor 	Disease	high-grade			NULL		0	NULL	NULL	NULL	NULL	NULL	Nocardia brain abscess mimicking high-grade necrotic tumor on perfusion MRI .	manualset1
80436	1	377259	7	NULL	NULL	0	NULL	Nocturia	Disease		common symptom in 					elderly	PersonGroup				NULL		0	NULL	NULL	NULL	NULL	NULL	Nocturia is a common symptom in the elderly , which profoundly influences general health and quality of life .	manualset1
80437	2	377259	7	NULL	NULL	NULL	NULL	statement 1	Process		influences		profoundly			general health	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nocturia is a common symptom in the elderly , which profoundly influences general health and quality of life .	manualset1
80438	3	377259	7	NULL	NULL	0	NULL	statement 1	Process		influences		profoundly			quality of life	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nocturia is a common symptom in the elderly , which profoundly influences general health and quality of life .	manualset1
80441	1	377260	7	NULL	NULL	0	NULL	Noggin 	Protein		recruits					mesoderm progenitors	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Noggin recruits mesoderm progenitors from the dorsal aorta to a skeletal myogenic fate .	manualset1
80444	2	377260	7	NULL	NULL	0	NULL	statement 1	Process		occur from					dorsal aorta	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Noggin recruits mesoderm progenitors from the dorsal aorta to a skeletal myogenic fate .	manualset1
80445	3	377260	7	NULL	NULL	0	NULL	statement 1	Process		occur to					skeletal myogenic fate	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Noggin recruits mesoderm progenitors from the dorsal aorta to a skeletal myogenic fate .	manualset1
80446	4	377260	7	NULL	NULL	0	NULL	statement 2	Process		occur along with					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Noggin recruits mesoderm progenitors from the dorsal aorta to a skeletal myogenic fate .	manualset1
80447	1	377261	7	NULL	NULL	0	NULL	Nogo-B 	Protein		phosphorylated by			Ser107		MAPKAP-K2	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	Nogo-B is phosphorylated at Ser107 in vitro by MAPKAP-K2 ( MAPK ( mitogen-activated protein kinase ) - activated protein kinase-2 ) or MAPKAP-K3 , but not by other protein kinases that are known to be activated by SAPK2a/p38a .	manualset1
80448	2	377261	7	NULL	NULL	0	NULL	Nogo-B 	Protein		phosphorylated by			Ser107		MAPKAP-K3	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	Nogo-B is phosphorylated at Ser107 in vitro by MAPKAP-K2 ( MAPK ( mitogen-activated protein kinase ) - activated protein kinase-2 ) or MAPKAP-K3 , but not by other protein kinases that are known to be activated by SAPK2a/p38a .	manualset1
80449	3	377261	7	NULL	NULL	0	NULL	MAPKAP-K2	Protein		is					( MAPK ( mitogen-activated protein kinase ) - activated protein kinase-2 )	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	Nogo-B is phosphorylated at Ser107 in vitro by MAPKAP-K2 ( MAPK ( mitogen-activated protein kinase ) - activated protein kinase-2 ) or MAPKAP-K3 , but not by other protein kinases that are known to be activated by SAPK2a/p38a .	manualset1
80450	4	377261	7	NULL	NULL	0	NULL	SAPK2a/p38a	Protein		activate					protein kinases	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	Nogo-B is phosphorylated at Ser107 in vitro by MAPKAP-K2 ( MAPK ( mitogen-activated protein kinase ) - activated protein kinase-2 ) or MAPKAP-K3 , but not by other protein kinases that are known to be activated by SAPK2a/p38a .	manualset1
80451	5	377261	7	NULL	NULL	0	NULL	statement 4	Process		does not phosphorylate					Nogo-B	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	Nogo-B is phosphorylated at Ser107 in vitro by MAPKAP-K2 ( MAPK ( mitogen-activated protein kinase ) - activated protein kinase-2 ) or MAPKAP-K3 , but not by other protein kinases that are known to be activated by SAPK2a/p38a .	manualset1
80452	6	377261	7	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nogo-B is phosphorylated at Ser107 in vitro by MAPKAP-K2 ( MAPK ( mitogen-activated protein kinase ) - activated protein kinase-2 ) or MAPKAP-K3 , but not by other protein kinases that are known to be activated by SAPK2a/p38a .	manualset1
80455	1	377264	7	NULL	NULL	0	NULL	( 3H ) dopamine	NonProteinOrNucleicAcidChemical		displaced by					( 1H ) dopamine	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Nomifensine , benztropine , PCP and amphetamine also inhibited the displacement of ( 3H ) dopamine by ( 1H ) dopamine at concentrations which have been shown previously to inhibit the uptake of ( 3H ) dopamine , suggesting that the mechanism behind displacement and uptake are very similar .	manualset1
80456	2	377264	7	NULL	NULL	0	NULL	Nomifensine	NonProteinOrNucleicAcidChemical		inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nomifensine , benztropine , PCP and amphetamine also inhibited the displacement of ( 3H ) dopamine by ( 1H ) dopamine at concentrations which have been shown previously to inhibit the uptake of ( 3H ) dopamine , suggesting that the mechanism behind displacement and uptake are very similar .	manualset1
80457	3	377264	7	NULL	NULL	0	NULL	benztropine	NonProteinOrNucleicAcidChemical		inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nomifensine , benztropine , PCP and amphetamine also inhibited the displacement of ( 3H ) dopamine by ( 1H ) dopamine at concentrations which have been shown previously to inhibit the uptake of ( 3H ) dopamine , suggesting that the mechanism behind displacement and uptake are very similar .	manualset1
80458	4	377264	7	NULL	NULL	0	NULL	PCP	NonProteinOrNucleicAcidChemical		inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nomifensine , benztropine , PCP and amphetamine also inhibited the displacement of ( 3H ) dopamine by ( 1H ) dopamine at concentrations which have been shown previously to inhibit the uptake of ( 3H ) dopamine , suggesting that the mechanism behind displacement and uptake are very similar .	manualset1
80459	5	377264	7	NULL	NULL	0	NULL	amphetamine	NonProteinOrNucleicAcidChemical		inhibit					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nomifensine , benztropine , PCP and amphetamine also inhibited the displacement of ( 3H ) dopamine by ( 1H ) dopamine at concentrations which have been shown previously to inhibit the uptake of ( 3H ) dopamine , suggesting that the mechanism behind displacement and uptake are very similar .	manualset1
80460	6	377264	7	NULL	NULL	0	NULL	Nomifensine	NonProteinOrNucleicAcidChemical		inhibit					( 3H ) dopamine	NonProteinOrNucleicAcidChemical	uptake of			NULL		0	NULL	NULL	NULL	NULL	NULL	Nomifensine , benztropine , PCP and amphetamine also inhibited the displacement of ( 3H ) dopamine by ( 1H ) dopamine at concentrations which have been shown previously to inhibit the uptake of ( 3H ) dopamine , suggesting that the mechanism behind displacement and uptake are very similar .	manualset1
80461	7	377264	7	NULL	NULL	0	NULL	benztropine	NonProteinOrNucleicAcidChemical		inhibit					( 3H ) dopamine	NonProteinOrNucleicAcidChemical	uptake of			NULL		0	NULL	NULL	NULL	NULL	NULL	Nomifensine , benztropine , PCP and amphetamine also inhibited the displacement of ( 3H ) dopamine by ( 1H ) dopamine at concentrations which have been shown previously to inhibit the uptake of ( 3H ) dopamine , suggesting that the mechanism behind displacement and uptake are very similar .	manualset1
80462	8	377264	7	NULL	NULL	0	NULL	PCP	NonProteinOrNucleicAcidChemical		inhibit					( 3H ) dopamine	NonProteinOrNucleicAcidChemical	uptake of			NULL		0	NULL	NULL	NULL	NULL	NULL	Nomifensine , benztropine , PCP and amphetamine also inhibited the displacement of ( 3H ) dopamine by ( 1H ) dopamine at concentrations which have been shown previously to inhibit the uptake of ( 3H ) dopamine , suggesting that the mechanism behind displacement and uptake are very similar .	manualset1
80463	9	377264	7	NULL	NULL	NULL	NULL	amphetamine	NonProteinOrNucleicAcidChemical		inhibit					( 3H ) dopamine	NonProteinOrNucleicAcidChemical	uptake of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nomifensine , benztropine , PCP and amphetamine also inhibited the displacement of ( 3H ) dopamine by ( 1H ) dopamine at concentrations which have been shown previously to inhibit the uptake of ( 3H ) dopamine , suggesting that the mechanism behind displacement and uptake are very similar .	manualset1
80464	10	377264	7	NULL	NULL	0	NULL	statement 2	Process		is similar to					statement 6	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nomifensine , benztropine , PCP and amphetamine also inhibited the displacement of ( 3H ) dopamine by ( 1H ) dopamine at concentrations which have been shown previously to inhibit the uptake of ( 3H ) dopamine , suggesting that the mechanism behind displacement and uptake are very similar .	manualset1
80465	11	377264	7	NULL	NULL	0	NULL	statement 3	Process		is similar to					statement 7	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nomifensine , benztropine , PCP and amphetamine also inhibited the displacement of ( 3H ) dopamine by ( 1H ) dopamine at concentrations which have been shown previously to inhibit the uptake of ( 3H ) dopamine , suggesting that the mechanism behind displacement and uptake are very similar .	manualset1
80466	12	377264	7	NULL	NULL	0	NULL	statement 4	Process		is similar to					statement 8	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nomifensine , benztropine , PCP and amphetamine also inhibited the displacement of ( 3H ) dopamine by ( 1H ) dopamine at concentrations which have been shown previously to inhibit the uptake of ( 3H ) dopamine , suggesting that the mechanism behind displacement and uptake are very similar .	manualset1
80467	13	377264	7	NULL	NULL	0	NULL	statement 5	Process		is similar to					statement 9	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nomifensine , benztropine , PCP and amphetamine also inhibited the displacement of ( 3H ) dopamine by ( 1H ) dopamine at concentrations which have been shown previously to inhibit the uptake of ( 3H ) dopamine , suggesting that the mechanism behind displacement and uptake are very similar .	manualset1
80468	1	377268	7	NULL	NULL	0	NULL	2-deoxy-D-glucose	NonProteinOrNucleicAcidChemical		induce		Non-hypoxic			HIF-3alpha	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	Non-hypoxic induction of HIF-3alpha by 2-deoxy-D-glucose and insulin .	manualset1
80469	2	377268	7	NULL	NULL	0	NULL	insulin	Protein		induce		Non-hypoxic			HIF-3alpha	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	Non-hypoxic induction of HIF-3alpha by 2-deoxy-D-glucose and insulin .	manualset1
80470	1	377270	7	NULL	NULL	NULL	NULL	Non-invasive liver iron	NonProteinOrNucleicAcidChemical	quantification of	diagnostic parameter for		new			hereditary hemochromatosis	Disease				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Non-invasive liver iron quantification by SQUID-biosusceptometry and serum ferritin iron as new diagnostic parameters in hereditary hemochromatosis .	manualset1
80471	2	377270	7	NULL	NULL	0	NULL	serum ferritin iron	NonProteinOrNucleicAcidChemical		diagnostic parameter for					hereditary hemochromatosis	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	Non-invasive liver iron quantification by SQUID-biosusceptometry and serum ferritin iron as new diagnostic parameters in hereditary hemochromatosis .	manualset1
80472	1	377271	7	NULL	NULL	0	NULL	Non-invasive ventilation	MedicalProcedure		given in					amyotrophic lateral sclerosis	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	Non-invasive ventilation in amyotrophic lateral sclerosis : a 10 year population based study .	manualset1
80473	1	377272	7	NULL	NULL	0	NULL	Non-necrotizing heparin	Protein		induce					skin lesions	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Non-necrotizing heparin-induced skin lesions and the 4T 's score .	manualset1
80474	1	377273	7	NULL	NULL	0	NULL	Non-nucleoside reverse transcriptase inhibitors	NonProteinOrNucleicAcidChemical		used in					new therapeutic regimens	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Non-nucleoside reverse transcriptase inhibitors can be used in new therapeutic regimens .	manualset1
80475	1	377276	7	NULL	NULL	0	NULL	Non-steroid anti-inflammatory drug therapy	MedicalProcedure		used in					orthopedics	MedicalProcedureOrDevice				NULL		0	NULL	NULL	NULL	NULL	NULL	Non-steroid anti-inflammatory drug therapy in various fields -- orthopedics ) .	manualset1
80476	1	377277	7	NULL	NULL	NULL	NULL	ibuprofen	NonProteinOrNucleicAcidChemical		induce					apoptosis	Process				NULL	human leukemic cells in vitro	NULL	NULL	NULL	NULL	NULL	NULL	Non-steroidal anti-inflammatory agent ibuprofen-induced apoptosis , cell necrosis and cell cycle alterations in human leukemic cells in vitro .	manualset1
80477	2	377277	7	NULL	NULL	NULL	NULL	ibuprofen	NonProteinOrNucleicAcidChemical		induce					cell necrosis	Process				NULL	human leukemic cells in vitro	NULL	NULL	NULL	NULL	NULL	NULL	Non-steroidal anti-inflammatory agent ibuprofen-induced apoptosis , cell necrosis and cell cycle alterations in human leukemic cells in vitro .	manualset1
80478	3	377277	7	NULL	NULL	NULL	NULL	ibuprofen	NonProteinOrNucleicAcidChemical		induce					cell cycle alterations	Process				NULL	human leukemic cells in vitro	NULL	NULL	NULL	NULL	NULL	NULL	Non-steroidal anti-inflammatory agent ibuprofen-induced apoptosis , cell necrosis and cell cycle alterations in human leukemic cells in vitro .	manualset1
80479	4	377277	7	NULL	NULL	0	NULL	ibuprofen	NonProteinOrNucleicAcidChemical		is a type of					Non-steroidal anti-inflammatory agent	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Non-steroidal anti-inflammatory agent ibuprofen-induced apoptosis , cell necrosis and cell cycle alterations in human leukemic cells in vitro .	manualset1
80480	1	377280	7	NULL	NULL	0	NULL	Nonablative skin remodeling	MedicalProcedure		option for					skin rejuvenation	MedicalProcedure	patients who demand a noninvasive approach			NULL		0	NULL	NULL	NULL	NULL	NULL	Nonablative skin remodeling has become an attractive option for patients whose lifestyles demand a noninvasive approach to skin rejuvenation .	manualset1
80595	1	377282	7	NULL	NULL	NULL	NULL	NANC	Process		demonstrated in					animal urinary bladder	BodyPart				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nonadrenergic , noncholinergic ( NANC ) contraction has been demonstrated in animal urinary bladder .	manualset1
80597	2	377282	7	NULL	NULL	0	NULL	NANC	Process		is					Nonadrenergic , noncholinergic contraction	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nonadrenergic , noncholinergic ( NANC ) contraction has been demonstrated in animal urinary bladder .	manualset1
80598	1	377284	7	NULL	NULL	0	NULL	benzoyl-CoA	NonProteinOrNucleicAcidChemical		converted to		anoxic			Nonaromatic products 	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Nonaromatic products from anoxic conversion of benzoyl-CoA with benzoyl-CoA reductase and cyclohexa-1 ,5 - diene-1-carbonyl-CoA hydratase .	manualset1
80599	2	377284	7	NULL	NULL	0	NULL	statement 1	Process		in presence with					benzoyl-CoA reductase	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	Nonaromatic products from anoxic conversion of benzoyl-CoA with benzoyl-CoA reductase and cyclohexa-1 ,5 - diene-1-carbonyl-CoA hydratase .	manualset1
80600	3	377284	7	NULL	NULL	NULL	NULL	statement 1	Process		in presence with					cyclohexa-1 ,5 - diene-1-carbonyl-CoA hydratase	Protein				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nonaromatic products from anoxic conversion of benzoyl-CoA with benzoyl-CoA reductase and cyclohexa-1 ,5 - diene-1-carbonyl-CoA hydratase .	manualset1
80601	1	377285	7	NULL	NULL	0	NULL	Nonbacterial meningitis	Disease		not detected		readily			clinically	MedicalProcedure				NULL		0	NULL	NULL	NULL	NULL	NULL	Nonbacterial meningitis can not be as readily detected clinically .	manualset1
80613	1	377286	7	NULL	NULL	0	NULL	Nonbacterial thrombotic endocarditis	Disease		occur with					malignant neoplastic diseases	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	Nonbacterial thrombotic endocarditis in patients with malignant neoplastic diseases .	manualset1
80614	1	377292	7	NULL	NULL	NULL	NULL	`` C. upsaliensis '' strains	Organism		not agglutinated with					 C. jejuni	Organism	antisera against heat-labile antigens from			NULL		NULL	NULL	NULL	NULL	NULL	NULL	None of the `` C. upsaliensis '' strains could be agglutinated with antisera against heat-labile antigens from C. jejuni , C. coli , or C. laridis .	manualset1
80615	2	377292	7	NULL	NULL	NULL	NULL	`` C. upsaliensis '' strains	Organism		not agglutinated with					 C. coli	Organism	antisera against heat-labile antigens from			NULL		NULL	NULL	NULL	NULL	NULL	NULL	None of the `` C. upsaliensis '' strains could be agglutinated with antisera against heat-labile antigens from C. jejuni , C. coli , or C. laridis .	manualset1
80616	3	377292	7	NULL	NULL	0	NULL	`` C. upsaliensis '' strains	Organism		not agglutinated with					 C. laridis	Organism	antisera against heat-labile antigens from			NULL		0	NULL	NULL	NULL	NULL	NULL	None of the `` C. upsaliensis '' strains could be agglutinated with antisera against heat-labile antigens from C. jejuni , C. coli , or C. laridis .	manualset1
80617	1	377296	7	NULL	NULL	NULL	NULL	lymphoma	Disease	mice without	shows					sIL-2R	Protein	detectable human			NULL		NULL	NULL	NULL	NULL	NULL	NULL	None of the control mice without lymphoma or with human nonlymphoid tumors ( prostatic carcinoma , ovarian carcinoma , and glioblastoma multiforme ) showed detectable human sIL-2R .	manualset1
80618	2	377296	7	NULL	NULL	0	NULL	prostatic carcinoma	Disease	mice with human	shows					sIL-2R	Protein	detectable human			NULL		0	NULL	NULL	NULL	NULL	NULL	None of the control mice without lymphoma or with human nonlymphoid tumors ( prostatic carcinoma , ovarian carcinoma , and glioblastoma multiforme ) showed detectable human sIL-2R .	manualset1
80619	3	377296	7	NULL	NULL	0	NULL	ovarian carcinoma	Disease	mice with human	shows					sIL-2R	Protein	detectable human			NULL		0	NULL	NULL	NULL	NULL	NULL	None of the control mice without lymphoma or with human nonlymphoid tumors ( prostatic carcinoma , ovarian carcinoma , and glioblastoma multiforme ) showed detectable human sIL-2R .	manualset1
80620	4	377296	7	NULL	NULL	NULL	NULL	glioblastoma multiforme	Disease	mice with human	shows					sIL-2R	Protein	detectable human			NULL		NULL	NULL	NULL	NULL	NULL	NULL	None of the control mice without lymphoma or with human nonlymphoid tumors ( prostatic carcinoma , ovarian carcinoma , and glioblastoma multiforme ) showed detectable human sIL-2R .	manualset1
80621	5	377296	7	NULL	NULL	0	NULL	prostatic carcinoma	Disease		is a type of					nonlymphoid tumors	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	None of the control mice without lymphoma or with human nonlymphoid tumors ( prostatic carcinoma , ovarian carcinoma , and glioblastoma multiforme ) showed detectable human sIL-2R .	manualset1
80622	6	377296	7	NULL	NULL	0	NULL	ovarian carcinoma	Disease		is a type of					nonlymphoid tumors	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	None of the control mice without lymphoma or with human nonlymphoid tumors ( prostatic carcinoma , ovarian carcinoma , and glioblastoma multiforme ) showed detectable human sIL-2R .	manualset1
80623	7	377296	7	NULL	NULL	NULL	NULL	glioblastoma multiforme	Disease		is a type of					nonlymphoid tumors	Protein				NULL		NULL	NULL	NULL	NULL	NULL	NULL	None of the control mice without lymphoma or with human nonlymphoid tumors ( prostatic carcinoma , ovarian carcinoma , and glioblastoma multiforme ) showed detectable human sIL-2R .	manualset1
80624	1	377301	7	NULL	NULL	0	NULL	pFSH-PVP treatments 	MedicalProcedure		not effective in					superovulation	Process	inducing			NULL		0	NULL	NULL	NULL	NULL	NULL	None of the pFSH-PVP treatments were effective in inducing superovulation .	manualset1
80626	1	377307	7	NULL	NULL	0	NULL	endogenous compounds	NonProteinOrNucleicAcidChemical		bind					Na + , K + - ATPase	Protein		cardiac glycoside binding site		NULL		0	NULL	NULL	NULL	NULL	NULL	None of these endogenous compounds has been shown conclusively to modulate sodium pump activity by binding to the cardiac glycoside binding site on Na + , K + - ATPase .	manualset1
80628	2	377307	7	NULL	NULL	0	NULL	statement 1	Process		does not modulate					sodium pump activity	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	None of these endogenous compounds has been shown conclusively to modulate sodium pump activity by binding to the cardiac glycoside binding site on Na + , K + - ATPase .	manualset1
80638	1	377312	7	NULL	NULL	0	NULL	protein C	Protein	Ser360Ala-activated 	shows					Nonenzymatic anticoagulant activity	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nonenzymatic anticoagulant activity of the mutant serine protease Ser360Ala-activated protein C mediated by factor Va.	manualset1
80639	2	377312	7	NULL	NULL	0	NULL	statement 1	Process		mediated by					factor Va	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	Nonenzymatic anticoagulant activity of the mutant serine protease Ser360Ala-activated protein C mediated by factor Va.	manualset1
80640	3	377312	7	NULL	NULL	0	NULL	 protein C	Protein	Ser360Ala-activated 	is a type of					mutant serine protease	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	Nonenzymatic anticoagulant activity of the mutant serine protease Ser360Ala-activated protein C mediated by factor Va.	manualset1
80641	1	377313	7	NULL	NULL	0	NULL	oxygen derivatives 	NonProteinOrNucleicAcidChemical	reduced	hydroxylation of		nonenzymatic			proline	AminoAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	Nonenzymatic hydroxylations of proline and lysine by reduced oxygen derivatives .	manualset1
80642	2	377313	7	NULL	NULL	0	NULL	oxygen derivatives 	NonProteinOrNucleicAcidChemical	reduced	hydroxylation of		nonenzymatic			lysine	AminoAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	Nonenzymatic hydroxylations of proline and lysine by reduced oxygen derivatives .	manualset1
80643	1	377314	7	NULL	NULL	0	NULL	short-chain phospholipids	NonProteinOrNucleicAcidChemical		activate		Nonessentially			phosphatidylinositol-specific phospholipase C	Protein	bacterial			NULL		0	NULL	NULL	NULL	NULL	NULL	Nonessential activation and competitive inhibition of bacterial phosphatidylinositol-specific phospholipase C by short-chain phospholipids and analogs .	manualset1
80644	2	377314	7	NULL	NULL	0	NULL	short-chain phospholipids	NonProteinOrNucleicAcidChemical		inhibit		competitively			phosphatidylinositol-specific phospholipase C	Protein	bacterial			NULL		0	NULL	NULL	NULL	NULL	NULL	Nonessential activation and competitive inhibition of bacterial phosphatidylinositol-specific phospholipase C by short-chain phospholipids and analogs .	manualset1
80645	3	377314	7	NULL	NULL	NULL	NULL	short-chain phospholipids	NonProteinOrNucleicAcidChemical	analogs of	activate		Nonessentially			phosphatidylinositol-specific phospholipase C	Protein	bacterial			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nonessential activation and competitive inhibition of bacterial phosphatidylinositol-specific phospholipase C by short-chain phospholipids and analogs .	manualset1
80646	4	377314	7	NULL	NULL	NULL	NULL	short-chain phospholipids	NonProteinOrNucleicAcidChemical	analogs of	inhibit		competitively			phosphatidylinositol-specific phospholipase C	Protein	bacterial			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nonessential activation and competitive inhibition of bacterial phosphatidylinositol-specific phospholipase C by short-chain phospholipids and analogs .	manualset1
80702	1	377321	7	NULL	NULL	0	NULL	Escherichia coli 	Organism	Nongrowing	produce					peptidoglycan	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Nongrowing Escherichia coli deprived of an essential amino acid continued to produce peptidoglycan at a rate approximately 30 % of that of growing cells .	manualset1
80703	2	377321	7	NULL	NULL	0	NULL	Escherichia coli 	Organism	Nongrowing	deprived of an					essential amino acid	AminoAcid				NULL		0	NULL	NULL	NULL	NULL	NULL	Nongrowing Escherichia coli deprived of an essential amino acid continued to produce peptidoglycan at a rate approximately 30 % of that of growing cells .	manualset1
80704	1	377322	7	NULL	NULL	0	NULL	Mre11 complex	Protein		mediate			globular domain		Nonhomologous end joining	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nonhomologous end joining , which is probably mediated by the globular domain of the Mre11 complex , was also severely impaired by alteration of the coiled-coil and hook domains , providing the first evidence of their influence on this process .	manualset1
80705	2	377322	7	NULL	NULL	0	NULL			alteration of	impair		severely	coiled-coil		statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nonhomologous end joining , which is probably mediated by the globular domain of the Mre11 complex , was also severely impaired by alteration of the coiled-coil and hook domains , providing the first evidence of their influence on this process .	manualset1
80707	3	377322	7	NULL	NULL	0	NULL			alteration of	impair		severely	hook domain		statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nonhomologous end joining , which is probably mediated by the globular domain of the Mre11 complex , was also severely impaired by alteration of the coiled-coil and hook domains , providing the first evidence of their influence on this process .	manualset1
80718	1	377325	7	NULL	NULL	NULL	NULL	Noninvasive genetic sampling	ResearchActivity		important to					wildlife populations	Organism	study			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Noninvasive genetic sampling approaches are becoming increasingly important to study wildlife populations .	manualset1
80864	1	377331	7	NULL	NULL	0	NULL	Nonneoplastic mucocutaneous lesions	MedicalFinding		occur in					organ transplant recipients	PersonGroup				NULL		0	NULL	NULL	NULL	NULL	NULL	Nonneoplastic mucocutaneous lesions in organ transplant recipients .	manualset1
80865	1	377335	7	NULL	NULL	0	NULL	sqt-1	Gene	Nonsense mutations of	cause					wild-type phenotypes	BiologicalProcess	not totally			NULL		0	NULL	NULL	NULL	NULL	NULL	Nonsense mutations of both sqt-1 and rol-6 cause nearly , but not totally , wild-type phenotypes .	manualset1
80866	2	377335	7	NULL	NULL	0	NULL	rol-6	Gene	Nonsense mutations of	cause					wild-type phenotypes	BiologicalProcess	not totally			NULL		0	NULL	NULL	NULL	NULL	NULL	Nonsense mutations of both sqt-1 and rol-6 cause nearly , but not totally , wild-type phenotypes .	manualset1
80867	1	377336	7	NULL	NULL	0	NULL	ketoconazole	NonProteinOrNucleicAcidChemical		inhibit		significantly			FK 506 metabolism	MolecularProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Nonspecific inhibitors of cytochrome P-450 , such as ketoconazole , itraconazole , fluconazole and SKF 525 A , and most of the cytochrome P-450 IIIA specific substrates used in this study significantly inhibited FK 506 metabolism .	manualset1
80868	2	377336	7	NULL	NULL	0	NULL	itraconazole	NonProteinOrNucleicAcidChemical		inhibit		significantly			FK 506 metabolism	MolecularProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Nonspecific inhibitors of cytochrome P-450 , such as ketoconazole , itraconazole , fluconazole and SKF 525 A , and most of the cytochrome P-450 IIIA specific substrates used in this study significantly inhibited FK 506 metabolism .	manualset1
80869	3	377336	7	NULL	NULL	0	NULL	fluconazole	NonProteinOrNucleicAcidChemical		inhibit		significantly			FK 506 metabolism	MolecularProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Nonspecific inhibitors of cytochrome P-450 , such as ketoconazole , itraconazole , fluconazole and SKF 525 A , and most of the cytochrome P-450 IIIA specific substrates used in this study significantly inhibited FK 506 metabolism .	manualset1
80870	4	377336	7	NULL	NULL	0	NULL	SKF 525 A	NonProteinOrNucleicAcidChemical		inhibit		significantly			FK 506 metabolism	MolecularProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Nonspecific inhibitors of cytochrome P-450 , such as ketoconazole , itraconazole , fluconazole and SKF 525 A , and most of the cytochrome P-450 IIIA specific substrates used in this study significantly inhibited FK 506 metabolism .	manualset1
80871	5	377336	7	NULL	NULL	0	NULL	cytochrome P-450 IIIA specific substrates	NonProteinOrNucleicAcidChemical		inhibit		significantly			FK 506 metabolism	MolecularProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Nonspecific inhibitors of cytochrome P-450 , such as ketoconazole , itraconazole , fluconazole and SKF 525 A , and most of the cytochrome P-450 IIIA specific substrates used in this study significantly inhibited FK 506 metabolism .	manualset1
80872	6	377336	7	NULL	NULL	0	NULL	ketoconazole	NonProteinOrNucleicAcidChemical		is a type of					cytochrome P-450	Protein	Nonspecific inhibitors of			NULL		0	NULL	NULL	NULL	NULL	NULL	Nonspecific inhibitors of cytochrome P-450 , such as ketoconazole , itraconazole , fluconazole and SKF 525 A , and most of the cytochrome P-450 IIIA specific substrates used in this study significantly inhibited FK 506 metabolism .	manualset1
80900	7	377336	7	NULL	NULL	0	NULL	itraconazole	NonProteinOrNucleicAcidChemical		is a type of					cytochrome P-450	Protein	Nonspecific inhibitors of			NULL		0	NULL	NULL	NULL	NULL	NULL	Nonspecific inhibitors of cytochrome P-450 , such as ketoconazole , itraconazole , fluconazole and SKF 525 A , and most of the cytochrome P-450 IIIA specific substrates used in this study significantly inhibited FK 506 metabolism .	manualset1
80901	8	377336	7	NULL	NULL	NULL	NULL	fluconazole	NonProteinOrNucleicAcidChemical		is a type of					cytochrome P-450	Protein	Nonspecific inhibitors of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nonspecific inhibitors of cytochrome P-450 , such as ketoconazole , itraconazole , fluconazole and SKF 525 A , and most of the cytochrome P-450 IIIA specific substrates used in this study significantly inhibited FK 506 metabolism .	manualset1
80902	9	377336	7	NULL	NULL	0	NULL	SKF 525 A	NonProteinOrNucleicAcidChemical		is a type of					cytochrome P-450	Protein	Nonspecific inhibitors of			NULL		0	NULL	NULL	NULL	NULL	NULL	Nonspecific inhibitors of cytochrome P-450 , such as ketoconazole , itraconazole , fluconazole and SKF 525 A , and most of the cytochrome P-450 IIIA specific substrates used in this study significantly inhibited FK 506 metabolism .	manualset1
80965	1	377338	7	NULL	NULL	0	NULL	NSAIDs	NonProteinOrNucleicAcidChemical		cause					acute diffuse injury	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Nonsteroidal anti-inflammatory drugs ( NSAIDs ) cause acute diffuse injury to the gastroduodenal mucosa , and also cause chronic focal ulcers that may bleed or perforate without warning symptoms .	manualset1
80966	2	377338	7	NULL	NULL	0	NULL	statement 1	Process		occur in					gastroduodenal mucosa	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Nonsteroidal anti-inflammatory drugs ( NSAIDs ) cause acute diffuse injury to the gastroduodenal mucosa , and also cause chronic focal ulcers that may bleed or perforate without warning symptoms .	manualset1
80967	3	377338	7	NULL	NULL	0	NULL	NSAIDs	NonProteinOrNucleicAcidChemical		cause					chronic focal ulcers	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Nonsteroidal anti-inflammatory drugs ( NSAIDs ) cause acute diffuse injury to the gastroduodenal mucosa , and also cause chronic focal ulcers that may bleed or perforate without warning symptoms .	manualset1
80968	4	377338	7	NULL	NULL	0	NULL	chronic focal ulcers	MedicalFinding		may					bleed	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Nonsteroidal anti-inflammatory drugs ( NSAIDs ) cause acute diffuse injury to the gastroduodenal mucosa , and also cause chronic focal ulcers that may bleed or perforate without warning symptoms .	manualset1
80969	5	377338	7	NULL	NULL	NULL	NULL	chronic focal ulcers	MedicalFinding		may					perforate	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nonsteroidal anti-inflammatory drugs ( NSAIDs ) cause acute diffuse injury to the gastroduodenal mucosa , and also cause chronic focal ulcers that may bleed or perforate without warning symptoms .	manualset1
80970	6	377338	7	NULL	NULL	NULL	NULL	statement 4	Process		occur without					warning symptoms	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nonsteroidal anti-inflammatory drugs ( NSAIDs ) cause acute diffuse injury to the gastroduodenal mucosa , and also cause chronic focal ulcers that may bleed or perforate without warning symptoms .	manualset1
80971	7	377338	7	NULL	NULL	0	NULL	statement 5	Process		occur without					warning symptoms	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Nonsteroidal anti-inflammatory drugs ( NSAIDs ) cause acute diffuse injury to the gastroduodenal mucosa , and also cause chronic focal ulcers that may bleed or perforate without warning symptoms .	manualset1
80972	8	377338	7	NULL	NULL	0	NULL	NSAIDs	NonProteinOrNucleicAcidChemical		is					Nonsteroidal anti-inflammatory drugs	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Nonsteroidal anti-inflammatory drugs ( NSAIDs ) cause acute diffuse injury to the gastroduodenal mucosa , and also cause chronic focal ulcers that may bleed or perforate without warning symptoms .	manualset1
80973	1	377339	7	NULL	NULL	0	NULL	Nonsteroidal anti-inflammatory drugs	NonProteinOrNucleicAcidChemical		associated with					hepatotoxicity	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Nonsteroidal anti-inflammatory drugs have been associated with hepatotoxicity in susceptible patients .	manualset1
80974	2	377339	7	NULL	NULL	0	NULL	statement 1	Process		occur in					susceptible patients	PersonGroup				NULL		0	NULL	NULL	NULL	NULL	NULL	Nonsteroidal anti-inflammatory drugs have been associated with hepatotoxicity in susceptible patients .	manualset1
80975	1	377342	7	NULL	NULL	0	NULL	1-stearoyllysophosphatidylcholine	NonProteinOrNucleicAcidChemical		dispersed in					water	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Nonsynchronicity phenomenon observed during the lamellar-micellar phase transitions of 1-stearoyllysophosphatidylcholine dispersed in water .	manualset1
80976	2	377342	7	NULL	NULL	0	NULL	Nonsynchronicity phenomenon	Process		observed during					statement 1	Process	lamellar-micellar phase transitions of			NULL		0	NULL	NULL	NULL	NULL	NULL	Nonsynchronicity phenomenon observed during the lamellar-micellar phase transitions of 1-stearoyllysophosphatidylcholine dispersed in water .	manualset1
80977	1	377344	7	NULL	NULL	0	NULL	SHP-2 phosphatase	Protein	Noonan syndrome/leukemia-associated gain-of-function mutations in	enhance					cell migration	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Noonan syndrome/leukemia-associated gain-of-function mutations in SHP-2 phosphatase ( PTPN11 ) enhance cell migration and angiogenesis .	manualset1
80978	2	377344	7	NULL	NULL	0	NULL	SHP-2 phosphatase	Protein	Noonan syndrome/leukemia-associated gain-of-function mutations in	enhance					angiogenesis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Noonan syndrome/leukemia-associated gain-of-function mutations in SHP-2 phosphatase ( PTPN11 ) enhance cell migration and angiogenesis .	manualset1
80979	3	377344	7	NULL	NULL	0	NULL	SHP-2 phosphatase	Protein		is					PTPN11	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	Noonan syndrome/leukemia-associated gain-of-function mutations in SHP-2 phosphatase ( PTPN11 ) enhance cell migration and angiogenesis .	manualset1
80980	1	377346	7	NULL	NULL	0	NULL	integrin	Protein		mediate					cell adhesiveness	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nor was the soluble peptide able to restore the loss of integrin-mediated cell adhesiveness to mini-laminin-332 after deletion of the gamma 2 chain C-terminus .	manualset1
80981	2	377346	7	NULL	NULL	NULL	NULL	soluble peptide	PartOfProtein		does not restore					statement 1	Process	loss of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nor was the soluble peptide able to restore the loss of integrin-mediated cell adhesiveness to mini-laminin-332 after deletion of the gamma 2 chain C-terminus .	manualset1
80982	3	377346	7	NULL	NULL	0	NULL	soluble peptide	PartOfProtein		does not restore					mini-laminin-332	Protein	loss of			NULL		0	NULL	NULL	NULL	NULL	NULL	Nor was the soluble peptide able to restore the loss of integrin-mediated cell adhesiveness to mini-laminin-332 after deletion of the gamma 2 chain C-terminus .	manualset1
80983	4	377346	7	NULL	NULL	0	NULL	statement 3	Process		occur after					mini-laminin-332	Protein	deletion of	gamma 2 chain C-terminus		NULL		0	NULL	NULL	NULL	NULL	NULL	Nor was the soluble peptide able to restore the loss of integrin-mediated cell adhesiveness to mini-laminin-332 after deletion of the gamma 2 chain C-terminus .	manualset1
80984	1	377347	7	NULL	NULL	0	NULL	BNI	NonProteinOrNucleicAcidChemical		does not block					dynorphin A	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Nor-BNI ( 4.9 nmol/mouse , i.c.v. ) did not block the effects of dynorphin A - ( 2-13 ) on the CO-induced impairment of learning and/or memory .	manualset1
80985	2	377347	7	NULL	NULL	0	NULL	CO	NonProteinOrNucleicAcidChemical		induce					learning	MentalProcess	impairment of			NULL		0	NULL	NULL	NULL	NULL	NULL	Nor-BNI ( 4.9 nmol/mouse , i.c.v. ) did not block the effects of dynorphin A - ( 2-13 ) on the CO-induced impairment of learning and/or memory .	manualset1
80986	3	377347	7	NULL	NULL	0	NULL	CO	NonProteinOrNucleicAcidChemical		induce					memory	MentalProcess	impairment of			NULL		0	NULL	NULL	NULL	NULL	NULL	Nor-BNI ( 4.9 nmol/mouse , i.c.v. ) did not block the effects of dynorphin A - ( 2-13 ) on the CO-induced impairment of learning and/or memory .	manualset1
80987	4	377347	7	NULL	NULL	0	NULL	statement 2	Process		is an alternative to					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nor-BNI ( 4.9 nmol/mouse , i.c.v. ) did not block the effects of dynorphin A - ( 2-13 ) on the CO-induced impairment of learning and/or memory .	manualset1
80988	5	377347	7	NULL	NULL	NULL	NULL	statement 1	Process		occur on					statement 2	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nor-BNI ( 4.9 nmol/mouse , i.c.v. ) did not block the effects of dynorphin A - ( 2-13 ) on the CO-induced impairment of learning and/or memory .	manualset1
80989	6	377347	7	NULL	NULL	0	NULL	statement 1	Process		occur on					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nor-BNI ( 4.9 nmol/mouse , i.c.v. ) did not block the effects of dynorphin A - ( 2-13 ) on the CO-induced impairment of learning and/or memory .	manualset1
80990	1	377348	7	NULL	NULL	0	NULL	Noradrenaline	NonProteinOrNucleicAcidChemical		release					Ca2+	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Noradrenaline and caffeine released 45Ca2 + from a cellular site in the aorta .	manualset1
80991	2	377348	7	NULL	NULL	0	NULL	caffeine	NonProteinOrNucleicAcidChemical		release					Ca2+	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Noradrenaline and caffeine released 45Ca2 + from a cellular site in the aorta .	manualset1
80992	3	377348	7	NULL	NULL	0	NULL	statement 1	Process		occur in					aorta	BodyPart	cellular site of			NULL		0	NULL	NULL	NULL	NULL	NULL	Noradrenaline and caffeine released 45Ca2 + from a cellular site in the aorta .	manualset1
80993	4	377348	7	NULL	NULL	0	NULL	statement 2	Process		occur in					aorta	BodyPart	cellular site of			NULL		0	NULL	NULL	NULL	NULL	NULL	Noradrenaline and caffeine released 45Ca2 + from a cellular site in the aorta .	manualset1
80994	1	377349	7	NULL	NULL	0	NULL	Norepinephrine	NonProteinOrNucleicAcidChemical		does not decrease					( methyl-14C ) choline	NonProteinOrNucleicAcidChemical	phosphorylation rate of			NULL		0	NULL	NULL	NULL	NULL	NULL	Norepinephrine ( plus propranolol ) does not decrease the uptake or phosphorylation rate of ( methyl-14C ) choline .	manualset1
80995	2	377349	7	NULL	NULL	NULL	NULL	Norepinephrine ( plus propranolol )	NonProteinOrNucleicAcidChemical		does not decrease					 ( methyl-14C ) choline	NonProteinOrNucleicAcidChemical	uptake of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Norepinephrine ( plus propranolol ) does not decrease the uptake or phosphorylation rate of ( methyl-14C ) choline .	manualset1
80996	1	377350	7	NULL	NULL	0	NULL	Norepinephrine	NonProteinOrNucleicAcidChemical		released from					sympathetic neurons	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Norepinephrine , released from sympathetic neurons , and epinephrine , released from the adrenal medulla , participate in a number of physiological processes including those that facilitate adaptation to stressful conditions .	manualset1
80997	2	377350	7	NULL	NULL	0	NULL	epinephrine	NonProteinOrNucleicAcidChemical		released from					adrenal medulla	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Norepinephrine , released from sympathetic neurons , and epinephrine , released from the adrenal medulla , participate in a number of physiological processes including those that facilitate adaptation to stressful conditions .	manualset1
80998	3	377350	7	NULL	NULL	NULL	NULL	statement 1	Process		participate in					physiological processes	BiologicalProcess				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Norepinephrine , released from sympathetic neurons , and epinephrine , released from the adrenal medulla , participate in a number of physiological processes including those that facilitate adaptation to stressful conditions .	manualset1
80999	4	377350	7	NULL	NULL	NULL	NULL	statement 2	Process		participate in					physiological processes	BiologicalProcess				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Norepinephrine , released from sympathetic neurons , and epinephrine , released from the adrenal medulla , participate in a number of physiological processes including those that facilitate adaptation to stressful conditions .	manualset1
81000	5	377350	7	NULL	NULL	NULL	NULL	physiological processes	BiologicalProcess		include					adaptation	BiologicalProcess				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Norepinephrine , released from sympathetic neurons , and epinephrine , released from the adrenal medulla , participate in a number of physiological processes including those that facilitate adaptation to stressful conditions .	manualset1
81001	6	377350	7	NULL	NULL	NULL	NULL	physiological processes	BiologicalProcess		include					stressful condition	BiologicalProcess				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Norepinephrine , released from sympathetic neurons , and epinephrine , released from the adrenal medulla , participate in a number of physiological processes including those that facilitate adaptation to stressful conditions .	manualset1
81002	7	377350	7	NULL	NULL	0	NULL	statement 1	Process		facilitate					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Norepinephrine , released from sympathetic neurons , and epinephrine , released from the adrenal medulla , participate in a number of physiological processes including those that facilitate adaptation to stressful conditions .	manualset1
81003	8	377350	7	NULL	NULL	0	NULL	statement 1	Process		facilitate					statement 6	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Norepinephrine , released from sympathetic neurons , and epinephrine , released from the adrenal medulla , participate in a number of physiological processes including those that facilitate adaptation to stressful conditions .	manualset1
81004	9	377350	7	NULL	NULL	0	NULL	statement 2	Process		facilitate					statement 5	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Norepinephrine , released from sympathetic neurons , and epinephrine , released from the adrenal medulla , participate in a number of physiological processes including those that facilitate adaptation to stressful conditions .	manualset1
81005	10	377350	7	NULL	NULL	0	NULL	statement 2	Process		facilitate					statement 6	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Norepinephrine , released from sympathetic neurons , and epinephrine , released from the adrenal medulla , participate in a number of physiological processes including those that facilitate adaptation to stressful conditions .	manualset1
81006	1	377351	7	NULL	NULL	0	NULL	Norepinephrine	NonProteinOrNucleicAcidChemical		induces					VEGF	Protein	expression of			NULL		0	NULL	NULL	NULL	NULL	NULL	Norepinephrine induces VEGF expression and angiogenesis by a hypoxia-inducible factor-1 protein-dependent mechanism .	manualset1
81007	2	377351	7	NULL	NULL	0	NULL	statement 1	Process		occur by					 hypoxia-inducible factor-1 protein-dependent mechanism	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Norepinephrine induces VEGF expression and angiogenesis by a hypoxia-inducible factor-1 protein-dependent mechanism .	manualset1
81008	3	377351	7	NULL	NULL	0	NULL	Norepinephrine	NonProteinOrNucleicAcidChemical		induces					angiogenesis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Norepinephrine induces VEGF expression and angiogenesis by a hypoxia-inducible factor-1 protein-dependent mechanism .	manualset1
81151	4	377351	7	NULL	NULL	0	NULL	statement 3	Process		occur by					hypoxia-inducible factor-1 protein-dependent mechanism	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Norepinephrine induces VEGF expression and angiogenesis by a hypoxia-inducible factor-1 protein-dependent mechanism .	manualset1
81152	1	377353	7	NULL	NULL	0	NULL	trisomy 8	Chromosome		sole abnormality of					 trisomy	MedicalFinding	frequent			NULL		0	NULL	NULL	NULL	NULL	NULL	Normal cytogenetics ( CN ) constitutes the single largest group , while trisomy 8 ( +8 ) as a sole abnormality is the most frequent trisomy .	manualset1
81153	1	377354	7	NULL	NULL	0	NULL	gastrin	Protein	normal fasting levels of	occur in					Zollinger-Ellison syndrome	MedicalFinding	patients with			NULL		0	NULL	NULL	NULL	NULL	NULL	Normal fasting gastrin levels do occur in patients with overt Zollinger-Ellison syndrome and should not deter further investigation if clinical suspicion of this syndrome is high .	manualset1
81154	1	377356	7	NULL	NULL	0	NULL	2 , 3-diphosphoglycerate	NonProteinOrNucleicAcidChemical	normal levels of	occur despite					chronic lung disease	MedicalFinding	severe hypoxemia of			NULL		0	NULL	NULL	NULL	NULL	NULL	Normal levels of 2 , 3-diphosphoglycerate in red cells despite severe hypoxemia of chronic lung disease .	manualset1
81155	2	377356	7	NULL	NULL	0	NULL	statement 1	Process		occur in					red cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Normal levels of 2 , 3-diphosphoglycerate in red cells despite severe hypoxemia of chronic lung disease .	manualset1
81156	1	377357	7	NULL	NULL	0	NULL	brain	BodyPart	normal maturation of mammalian	characterized by					glucose transport	Process	periods of limitation in			NULL		0	NULL	NULL	NULL	NULL	NULL	Normal maturation of the mammalian brain is characterized by periods of limitations in glucose transport capacity and increased use of alternative cerebral metabolic fuels such as lactate and ketone bodies , all of which are important during H/I and influence the development of energy failure .	manualset1
81157	2	377357	7	NULL	NULL	0	NULL	brain	BodyPart	normal maturation of mammalian	characterized by					lactate	NonProteinOrNucleicAcidChemical	increased use of			NULL		0	NULL	NULL	NULL	NULL	NULL	Normal maturation of the mammalian brain is characterized by periods of limitations in glucose transport capacity and increased use of alternative cerebral metabolic fuels such as lactate and ketone bodies , all of which are important during H/I and influence the development of energy failure .	manualset1
81158	3	377357	7	NULL	NULL	0	NULL	brain	BodyPart	normal maturation of mammalian	characterized by					ketone bodies	NonProteinOrNucleicAcidChemical	increased use of			NULL		0	NULL	NULL	NULL	NULL	NULL	Normal maturation of the mammalian brain is characterized by periods of limitations in glucose transport capacity and increased use of alternative cerebral metabolic fuels such as lactate and ketone bodies , all of which are important during H/I and influence the development of energy failure .	manualset1
81159	4	377357	7	NULL	NULL	0	NULL	lactate	NonProteinOrNucleicAcidChemical		is a type of					alternative cerebral metabolic fuel	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Normal maturation of the mammalian brain is characterized by periods of limitations in glucose transport capacity and increased use of alternative cerebral metabolic fuels such as lactate and ketone bodies , all of which are important during H/I and influence the development of energy failure .	manualset1
81161	5	377357	7	NULL	NULL	0	NULL	Ketone bodies	NonProteinOrNucleicAcidChemical		is a type of					alternative cerebral metabolic fuel	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Normal maturation of the mammalian brain is characterized by periods of limitations in glucose transport capacity and increased use of alternative cerebral metabolic fuels such as lactate and ketone bodies , all of which are important during H/I and influence the development of energy failure .	manualset1
81165	6	377357	7	NULL	NULL	0	NULL	lactate	NonProteinOrNucleicAcidChemical		important during					H/I	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Normal maturation of the mammalian brain is characterized by periods of limitations in glucose transport capacity and increased use of alternative cerebral metabolic fuels such as lactate and ketone bodies , all of which are important during H/I and influence the development of energy failure .	manualset1
81166	7	377357	7	NULL	NULL	0	NULL	ketone bodies	NonProteinOrNucleicAcidChemical		important during					H/I	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Normal maturation of the mammalian brain is characterized by periods of limitations in glucose transport capacity and increased use of alternative cerebral metabolic fuels such as lactate and ketone bodies , all of which are important during H/I and influence the development of energy failure .	manualset1
81167	8	377357	7	NULL	NULL	0	NULL	lactate	NonProteinOrNucleicAcidChemical		influence					energy failure	Process	development of			NULL		0	NULL	NULL	NULL	NULL	NULL	Normal maturation of the mammalian brain is characterized by periods of limitations in glucose transport capacity and increased use of alternative cerebral metabolic fuels such as lactate and ketone bodies , all of which are important during H/I and influence the development of energy failure .	manualset1
81169	9	377357	7	NULL	NULL	0	NULL	ketone bodies	NonProteinOrNucleicAcidChemical		influence					energy failure	Process	development of			NULL		0	NULL	NULL	NULL	NULL	NULL	Normal maturation of the mammalian brain is characterized by periods of limitations in glucose transport capacity and increased use of alternative cerebral metabolic fuels such as lactate and ketone bodies , all of which are important during H/I and influence the development of energy failure .	manualset1
81171	1	377359	7	NULL	NULL	0	NULL	cerebral blood flow 	BiologicalProcess		low in					newborn	PersonGroup	normal			NULL		0	NULL	NULL	NULL	NULL	NULL	Normal newborn cerebral blood flow is low ; fetal asphyxia at birth causes delayed cerebral hyperperfusion in the neonate .	manualset1
81172	2	377359	7	NULL	NULL	0	NULL	fetal asphyxia	MedicalFinding		cause					cerebral hyperperfusion	BiologicalProcess	delayed			NULL		0	NULL	NULL	NULL	NULL	NULL	Normal newborn cerebral blood flow is low ; fetal asphyxia at birth causes delayed cerebral hyperperfusion in the neonate .	manualset1
81173	3	377359	7	NULL	NULL	0	NULL	statement 2	Process		occur at					birth	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Normal newborn cerebral blood flow is low ; fetal asphyxia at birth causes delayed cerebral hyperperfusion in the neonate .	manualset1
81174	4	377359	7	NULL	NULL	0	NULL	statement 2	Process		occur in the					neonate	PersonGroup				NULL		0	NULL	NULL	NULL	NULL	NULL	Normal newborn cerebral blood flow is low ; fetal asphyxia at birth causes delayed cerebral hyperperfusion in the neonate .	manualset1
81175	1	377360	7	NULL	NULL	0	NULL	 platelets	BodyPart	Normal	have					NOS activity	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Normal platelets are known to have NOS activity , but little is known about NOS expression and NO production by platelets in patients with IPAH .	manualset1
81177	1	377361	7	NULL	NULL	0	NULL	left ventricle	BodyPart	Normal size	occur in					lethal hypoplastic left heart syndrome	MedicalFinding	antenatal scan			NULL		0	NULL	NULL	NULL	NULL	NULL	Normal size left ventricle on antenatal scan in lethal hypoplastic left heart syndrome .	manualset1
81178	1	377365	7	NULL	NULL	0	NULL	hemoglobin 	BodyPart	normalization of	does not have					cardiac structure	BodyPart	effect on			NULL		0	NULL	NULL	NULL	NULL	NULL	Normalization of hemoglobin in incident hemodialysis patients does not have a beneficial effect on cardiac structure , compared with partial correction .	manualset1
81180	2	377365	7	NULL	NULL	0	NULL	statement 1	Process		occur in					incident hemodialysis patients	PersonGroup				NULL		0	NULL	NULL	NULL	NULL	NULL	Normalization of hemoglobin in incident hemodialysis patients does not have a beneficial effect on cardiac structure , compared with partial correction .	manualset1
81182	1	377370	7	NULL	NULL	NULL	NULL	opioid receptor clones	Protein		expressed at			delta		low levels	Quantity				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Northern analyses with riboprobes derived from the delta and kappa opioid receptor clones indicate these sequences are expressed at low levels in human peripheral blood lymphocytes and in several human lymphoid cell lines .	manualset1
81183	2	377370	7	NULL	NULL	0	NULL	opioid receptor clones	Protein		expressed at			kappa		low levels	Quantity				NULL		0	NULL	NULL	NULL	NULL	NULL	Northern analyses with riboprobes derived from the delta and kappa opioid receptor clones indicate these sequences are expressed at low levels in human peripheral blood lymphocytes and in several human lymphoid cell lines .	manualset1
81184	3	377370	7	NULL	NULL	0	NULL	statement 1	Process		occur in					 peripheral blood lymphocytes	Cell	human			NULL		0	NULL	NULL	NULL	NULL	NULL	Northern analyses with riboprobes derived from the delta and kappa opioid receptor clones indicate these sequences are expressed at low levels in human peripheral blood lymphocytes and in several human lymphoid cell lines .	manualset1
81185	4	377370	7	NULL	NULL	0	NULL	statement 2	Process		occur in					peripheral blood lymphocytes	Cell	human			NULL		0	NULL	NULL	NULL	NULL	NULL	Northern analyses with riboprobes derived from the delta and kappa opioid receptor clones indicate these sequences are expressed at low levels in human peripheral blood lymphocytes and in several human lymphoid cell lines .	manualset1
81186	5	377370	7	NULL	NULL	NULL	NULL	statement 1	Process		occur in					lymphoid cell lines	Cell	human			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Northern analyses with riboprobes derived from the delta and kappa opioid receptor clones indicate these sequences are expressed at low levels in human peripheral blood lymphocytes and in several human lymphoid cell lines .	manualset1
81187	6	377370	7	NULL	NULL	0	NULL	statement 2	Process		occur in					lymphoid cell lines	Cell	human			NULL		0	NULL	NULL	NULL	NULL	NULL	Northern analyses with riboprobes derived from the delta and kappa opioid receptor clones indicate these sequences are expressed at low levels in human peripheral blood lymphocytes and in several human lymphoid cell lines .	manualset1
81188	1	377371	7	NULL	NULL	0	NULL	neugrin	Protein		expressed in		strongly			heart	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Northern analysis revealed that neugrin was strongly expressed in the heart , brain , and skeletal muscle , and m-neugrin in the liver , kidney , and brain .	manualset1
81189	2	377371	7	NULL	NULL	0	NULL	neugrin	Protein		expressed in		strongly			brain	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Northern analysis revealed that neugrin was strongly expressed in the heart , brain , and skeletal muscle , and m-neugrin in the liver , kidney , and brain .	manualset1
81190	3	377371	7	NULL	NULL	0	NULL	neugrin	Protein		expressed in		strongly			skeletal muscle	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Northern analysis revealed that neugrin was strongly expressed in the heart , brain , and skeletal muscle , and m-neugrin in the liver , kidney , and brain .	manualset1
81191	4	377371	7	NULL	NULL	0	NULL	 m-neugrin	Protein		expressed in					liver	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Northern analysis revealed that neugrin was strongly expressed in the heart , brain , and skeletal muscle , and m-neugrin in the liver , kidney , and brain .	manualset1
81192	5	377371	7	NULL	NULL	0	NULL	m-neugrin	Protein		expressed in					kidney	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Northern analysis revealed that neugrin was strongly expressed in the heart , brain , and skeletal muscle , and m-neugrin in the liver , kidney , and brain .	manualset1
81193	6	377371	7	NULL	NULL	0	NULL	m-neugrin	Protein		expressed in					brain	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Northern analysis revealed that neugrin was strongly expressed in the heart , brain , and skeletal muscle , and m-neugrin in the liver , kidney , and brain .	manualset1
81194	1	377372	7	NULL	NULL	NULL	NULL	Nogo-A	Protein		expressed in		predominantly			nervous system	BodyPart				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Northern and Western blot analysis indicated that Nogo-A is predominantly expressed in the nervous system with lower levels also present in testis and heart .	manualset1
81195	2	377372	7	NULL	NULL	0	NULL	Nogo-A	Protein		expressed in					testis	BodyPart	lower levels in			NULL		0	NULL	NULL	NULL	NULL	NULL	Northern and Western blot analysis indicated that Nogo-A is predominantly expressed in the nervous system with lower levels also present in testis and heart .	manualset1
81196	3	377372	7	NULL	NULL	0	NULL	Nogo-A	Protein		expressed in					heart	BodyPart	lower levels in			NULL		0	NULL	NULL	NULL	NULL	NULL	Northern and Western blot analysis indicated that Nogo-A is predominantly expressed in the nervous system with lower levels also present in testis and heart .	manualset1
81202	1	377377	7	NULL	NULL	0	NULL	11-9-1-4	Cell		express					galectin-3	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Not only did 11-9-1-4 express galectin-3 in the usual punctate pattern on its cell surface , it demonstrated a higher surface expression of alpha 6 beta 1 integrin compared to BT-549 .	manualset1
81204	2	377377	7	NULL	NULL	NULL	NULL	statement 1	Process		occur in the					cell surface	Cell	punctate pattern on			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Not only did 11-9-1-4 express galectin-3 in the usual punctate pattern on its cell surface , it demonstrated a higher surface expression of alpha 6 beta 1 integrin compared to BT-549 .	manualset1
81205	3	377377	7	NULL	NULL	0	NULL	11-9-1-4 	Cell		express					alpha 6 beta 1 integrin	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	Not only did 11-9-1-4 express galectin-3 in the usual punctate pattern on its cell surface , it demonstrated a higher surface expression of alpha 6 beta 1 integrin compared to BT-549 .	manualset1
81206	4	377377	7	NULL	NULL	0	NULL	BT-549	Cell		express					alpha 6 beta 1 integrin	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	Not only did 11-9-1-4 express galectin-3 in the usual punctate pattern on its cell surface , it demonstrated a higher surface expression of alpha 6 beta 1 integrin compared to BT-549 .	manualset1
81207	5	377377	7	NULL	NULL	0	NULL	statement 3	Process	expression of	is higher than					statement 4	Process	expression of			NULL		0	NULL	NULL	NULL	NULL	NULL	Not only did 11-9-1-4 express galectin-3 in the usual punctate pattern on its cell surface , it demonstrated a higher surface expression of alpha 6 beta 1 integrin compared to BT-549 .	manualset1
81201	1	377378	7	NULL	NULL	0	NULL	adult neurogenesis	Process		respond to					hippocampal damage 	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Not surprising , investigators of Alzheimer 's disease have also evaluated adult neurogenesis due to its responsiveness to hippocampal damage .	manualset1
81208	1	377379	7	NULL	NULL	0	NULL	ARD1	Protein		critical for					AR target genes	Gene	transcriptionally regulating			NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , ARD1 was critical for transcriptionally regulating a number of AR target genes that are involved in prostate tumorigenesis .	manualset1
81209	2	377379	7	NULL	NULL	0	NULL	AR target genes	Gene		involved in					prostate tumorigenesis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , ARD1 was critical for transcriptionally regulating a number of AR target genes that are involved in prostate tumorigenesis .	manualset1
81271	1	377381	7	NULL	NULL	NULL	NULL	HCV-JFH1 	Organism	 infection of	redistribute					G3BP1	Protein				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Notably , HCV-JFH1 infection also redistributed the stress granule components GTPase-activating protein ( SH3 domain ) - binding protein 1 ( G3BP1 ) , ataxin-2 ( ATX2 ) , and poly ( A ) - binding protein 1 ( PABP1 ) to the HCV production factory .	manualset1
81272	2	377381	7	NULL	NULL	0	NULL	HCV-JFH1 	Organism	infection of	redistribute					ATX2	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , HCV-JFH1 infection also redistributed the stress granule components GTPase-activating protein ( SH3 domain ) - binding protein 1 ( G3BP1 ) , ataxin-2 ( ATX2 ) , and poly ( A ) - binding protein 1 ( PABP1 ) to the HCV production factory .	manualset1
81273	3	377381	7	NULL	NULL	0	NULL	HCV-JFH1 	Organism	infection of	redistribute					PABP1	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , HCV-JFH1 infection also redistributed the stress granule components GTPase-activating protein ( SH3 domain ) - binding protein 1 ( G3BP1 ) , ataxin-2 ( ATX2 ) , and poly ( A ) - binding protein 1 ( PABP1 ) to the HCV production factory .	manualset1
81274	4	377381	7	NULL	NULL	0	NULL	statement 1	Process		redistribute to					HCV production factory	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , HCV-JFH1 infection also redistributed the stress granule components GTPase-activating protein ( SH3 domain ) - binding protein 1 ( G3BP1 ) , ataxin-2 ( ATX2 ) , and poly ( A ) - binding protein 1 ( PABP1 ) to the HCV production factory .	manualset1
81275	5	377381	7	NULL	NULL	0	NULL	statement 2	Process		redistribute to					HCV production factory	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , HCV-JFH1 infection also redistributed the stress granule components GTPase-activating protein ( SH3 domain ) - binding protein 1 ( G3BP1 ) , ataxin-2 ( ATX2 ) , and poly ( A ) - binding protein 1 ( PABP1 ) to the HCV production factory .	manualset1
81276	6	377381	7	NULL	NULL	0	NULL	statement 3	Process		redistribute to					HCV production factory	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , HCV-JFH1 infection also redistributed the stress granule components GTPase-activating protein ( SH3 domain ) - binding protein 1 ( G3BP1 ) , ataxin-2 ( ATX2 ) , and poly ( A ) - binding protein 1 ( PABP1 ) to the HCV production factory .	manualset1
81277	7	377381	7	NULL	NULL	0	NULL	G3BP1	Protein		is a type of					stress granule component	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , HCV-JFH1 infection also redistributed the stress granule components GTPase-activating protein ( SH3 domain ) - binding protein 1 ( G3BP1 ) , ataxin-2 ( ATX2 ) , and poly ( A ) - binding protein 1 ( PABP1 ) to the HCV production factory .	manualset1
81278	8	377381	7	NULL	NULL	0	NULL	ATX2	Protein		is a type of					stress granule component	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , HCV-JFH1 infection also redistributed the stress granule components GTPase-activating protein ( SH3 domain ) - binding protein 1 ( G3BP1 ) , ataxin-2 ( ATX2 ) , and poly ( A ) - binding protein 1 ( PABP1 ) to the HCV production factory .	manualset1
81279	9	377381	7	NULL	NULL	0	NULL	PABP1	Protein		is a type of					stress granule component	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , HCV-JFH1 infection also redistributed the stress granule components GTPase-activating protein ( SH3 domain ) - binding protein 1 ( G3BP1 ) , ataxin-2 ( ATX2 ) , and poly ( A ) - binding protein 1 ( PABP1 ) to the HCV production factory .	manualset1
81281	10	377381	7	NULL	NULL	0	NULL	G3BP1	Protein		is					GTPase-activating protein ( SH3 domain ) - binding protein 1	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , HCV-JFH1 infection also redistributed the stress granule components GTPase-activating protein ( SH3 domain ) - binding protein 1 ( G3BP1 ) , ataxin-2 ( ATX2 ) , and poly ( A ) - binding protein 1 ( PABP1 ) to the HCV production factory .	manualset1
81282	11	377381	7	NULL	NULL	0	NULL	ATX2	Protein		is					ataxin-2	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , HCV-JFH1 infection also redistributed the stress granule components GTPase-activating protein ( SH3 domain ) - binding protein 1 ( G3BP1 ) , ataxin-2 ( ATX2 ) , and poly ( A ) - binding protein 1 ( PABP1 ) to the HCV production factory .	manualset1
81283	12	377381	7	NULL	NULL	0	NULL	PABP1	Protein		is					poly ( A ) - binding protein 1	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , HCV-JFH1 infection also redistributed the stress granule components GTPase-activating protein ( SH3 domain ) - binding protein 1 ( G3BP1 ) , ataxin-2 ( ATX2 ) , and poly ( A ) - binding protein 1 ( PABP1 ) to the HCV production factory .	manualset1
81284	1	377382	7	NULL	NULL	0	NULL	HDAC inhibitors	NonProteinOrNucleicAcidChemical		led to					HDAC4	Protein	degradation of			NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , HDAC inhibitors led to noticeable HDAC4 degradation , which was effectively prevented by MG132 .	manualset1
81285	2	377382	7	NULL	NULL	0	NULL	MG132	NonProteinOrNucleicAcidChemical		prevent		effectively			statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , HDAC inhibitors led to noticeable HDAC4 degradation , which was effectively prevented by MG132 .	manualset1
81286	1	377386	7	NULL	NULL	0	NULL	heparanase	Protein		stimulate					macrophage	Cell	activation of			NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , heparanase stimulates macrophage activation , while macrophages induce production and activation of latent heparanase contributed by the colon epithelium , together generating a vicious cycle that powers colitis and the associated tumorigenesis .	manualset1
81287	2	377386	7	NULL	NULL	0	NULL	macrophages 	Cell		induce					latent heparanase	Protein	production of			NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , heparanase stimulates macrophage activation , while macrophages induce production and activation of latent heparanase contributed by the colon epithelium , together generating a vicious cycle that powers colitis and the associated tumorigenesis .	manualset1
81288	3	377386	7	NULL	NULL	0	NULL	macrophages 	Cell		induce					latent heparanase	Protein	activation of			NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , heparanase stimulates macrophage activation , while macrophages induce production and activation of latent heparanase contributed by the colon epithelium , together generating a vicious cycle that powers colitis and the associated tumorigenesis .	manualset1
81289	4	377386	7	NULL	NULL	0	NULL	statement 2	Process		contributed by					colon epithelium	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , heparanase stimulates macrophage activation , while macrophages induce production and activation of latent heparanase contributed by the colon epithelium , together generating a vicious cycle that powers colitis and the associated tumorigenesis .	manualset1
81290	5	377386	7	NULL	NULL	0	NULL	statement 3	Process		contributed by					colon epithelium	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , heparanase stimulates macrophage activation , while macrophages induce production and activation of latent heparanase contributed by the colon epithelium , together generating a vicious cycle that powers colitis and the associated tumorigenesis .	manualset1
81291	6	377386	7	NULL	NULL	0	NULL	statement 4	Process		generate					vicious cycle	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , heparanase stimulates macrophage activation , while macrophages induce production and activation of latent heparanase contributed by the colon epithelium , together generating a vicious cycle that powers colitis and the associated tumorigenesis .	manualset1
81292	7	377386	7	NULL	NULL	0	NULL	statement 5	Process		generate					vicious cycle	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , heparanase stimulates macrophage activation , while macrophages induce production and activation of latent heparanase contributed by the colon epithelium , together generating a vicious cycle that powers colitis and the associated tumorigenesis .	manualset1
81293	8	377386	7	NULL	NULL	0	NULL	statement 6	Process		powers					colitis	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , heparanase stimulates macrophage activation , while macrophages induce production and activation of latent heparanase contributed by the colon epithelium , together generating a vicious cycle that powers colitis and the associated tumorigenesis .	manualset1
81294	9	377386	7	NULL	NULL	0	NULL	statement 7	Process		powers					colitis	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , heparanase stimulates macrophage activation , while macrophages induce production and activation of latent heparanase contributed by the colon epithelium , together generating a vicious cycle that powers colitis and the associated tumorigenesis .	manualset1
81295	10	377386	7	NULL	NULL	0	NULL	statement 6	Process		powers					tumorigenesis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , heparanase stimulates macrophage activation , while macrophages induce production and activation of latent heparanase contributed by the colon epithelium , together generating a vicious cycle that powers colitis and the associated tumorigenesis .	manualset1
81296	11	377386	7	NULL	NULL	0	NULL	statement 7	Process		powers					tumorigenesis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , heparanase stimulates macrophage activation , while macrophages induce production and activation of latent heparanase contributed by the colon epithelium , together generating a vicious cycle that powers colitis and the associated tumorigenesis .	manualset1
81297	1	377388	7	NULL	NULL	0	NULL	neuronal protein	Protein		aggregates					huntingtin	Protein	mutated			NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , neuronal protein aggregates of mutated huntingtin , which is typical HD neuropathology , were not found within the transplanted fetal tissue .	manualset1
81298	2	377388	7	NULL	NULL	0	NULL	statement 1	Process		is a type of					typical HD neuropathology	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , neuronal protein aggregates of mutated huntingtin , which is typical HD neuropathology , were not found within the transplanted fetal tissue .	manualset1
81299	3	377388	7	NULL	NULL	0	NULL	statement 1	Process		not found within					 fetal tissue	BodyPart	transplanted			NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , neuronal protein aggregates of mutated huntingtin , which is typical HD neuropathology , were not found within the transplanted fetal tissue .	manualset1
81300	1	377391	7	NULL	NULL	0	NULL	Notch 	Protein		does not affect		overtly			cell cycle	Process	entry of			NULL		0	NULL	NULL	NULL	NULL	NULL	Notch does not overtly affect cell cycle entry or progression of CD4 ( + ) T cells .	manualset1
81301	2	377391	7	NULL	NULL	0	NULL	Notch	Protein		does not affect		overtly			CD4 ( + ) T cells	Cell	progression of			NULL		0	NULL	NULL	NULL	NULL	NULL	Notch does not overtly affect cell cycle entry or progression of CD4 ( + ) T cells .	manualset1
81366	1	377392	7	NULL	NULL	0	NULL	Notch	Protein		implicated as					myogenesis	Process	regulator of			NULL		0	NULL	NULL	NULL	NULL	NULL	Notch has also been implicated as a regulator of myogenesis , although its precise function there has remained controversial .	manualset1
81302	1	377393	7	NULL	NULL	0	NULL	Notch signaling	Process		is involved in					cell differentiation	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Notch signaling is involved in cell differentiation and patterning during morphogenesis .	manualset1
81303	2	377393	7	NULL	NULL	0	NULL	Notch signaling	Process		is involved in					patterning	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Notch signaling is involved in cell differentiation and patterning during morphogenesis .	manualset1
81304	3	377393	7	NULL	NULL	0	NULL	statement 1	Process		occur during					morphogenesis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Notch signaling is involved in cell differentiation and patterning during morphogenesis .	manualset1
81305	4	377393	7	NULL	NULL	0	NULL	statement 2	Process		occur during					morphogenesis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Notch signaling is involved in cell differentiation and patterning during morphogenesis .	manualset1
81306	3	377398	7	NULL	NULL	NULL	NULL	chronic stress	MentalProcess		impair					statement 1	BodyPart	development of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Noting that chronic stress or abuse in childhood can impair development of the brain region involved in learning and memory , the authors show how the extreme stress of being placed in an orphanage leads to abnormal brain development and decreased cognitive functioning .	manualset1
81307	5	377398	7	NULL	NULL	NULL	NULL	statement 3	Process		during					childhood	Duration				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Noting that chronic stress or abuse in childhood can impair development of the brain region involved in learning and memory , the authors show how the extreme stress of being placed in an orphanage leads to abnormal brain development and decreased cognitive functioning .	manualset1
81308	1	377398	7	NULL	NULL	0	NULL	brain region	BodyPart		involved in					learning	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Noting that chronic stress or abuse in childhood can impair development of the brain region involved in learning and memory , the authors show how the extreme stress of being placed in an orphanage leads to abnormal brain development and decreased cognitive functioning .	manualset1
81309	2	377398	7	NULL	NULL	0	NULL	brain region	BodyPart		involved in					memory	MentalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	Noting that chronic stress or abuse in childhood can impair development of the brain region involved in learning and memory , the authors show how the extreme stress of being placed in an orphanage leads to abnormal brain development and decreased cognitive functioning .	manualset1
81310	4	377398	7	NULL	NULL	0	NULL	chronic stress	MentalProcess		impair					statement 2	Protein	development of			NULL		0	NULL	NULL	NULL	NULL	NULL	Noting that chronic stress or abuse in childhood can impair development of the brain region involved in learning and memory , the authors show how the extreme stress of being placed in an orphanage leads to abnormal brain development and decreased cognitive functioning .	manualset1
81311	6	377398	7	NULL	NULL	NULL	NULL	statement 4	Process		during					childhood	Duration				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Noting that chronic stress or abuse in childhood can impair development of the brain region involved in learning and memory , the authors show how the extreme stress of being placed in an orphanage leads to abnormal brain development and decreased cognitive functioning .	manualset1
81312	1	377401	7	NULL	NULL	0	NULL	Novel 5 ' - norcarbocyclic adenine analogs	NonProteinOrNucleicAcidChemical		synthesized from					epichlorohydrin 5	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Novel 5 ' - norcarbocyclic adenine and guanine phosphonic acid analogs with 6 ' ,6 ' - difluorine moiety were designed and synthesized from commercially available epichlorohydrin 5 .	manualset1
81313	2	377401	7	NULL	NULL	0	NULL	guanine phosphonic acid analogs with 6 ' ,6 ' - difluorine moiety	NonProteinOrNucleicAcidChemical		synthesized from					epichlorohydrin 5	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Novel 5 ' - norcarbocyclic adenine and guanine phosphonic acid analogs with 6 ' ,6 ' - difluorine moiety were designed and synthesized from commercially available epichlorohydrin 5 .	manualset1
81314	1	377404	7	NULL	NULL	0	NULL	Novel calpain inhibitors	NonProteinOrNucleicAcidChemical		derived from					phenyl alanine aldehydes	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Novel calpain inhibitors derived from phenyl alanine aldehydes or ketoamides carrying a benzoyl residue were prepared and evaluated for their biological potency .	manualset1
81315	2	377404	7	NULL	NULL	0	NULL	Novel calpain inhibitors	NonProteinOrNucleicAcidChemical		derived from					phenyl alanine ketoamides	NonProteinOrNucleicAcidChemical	carrying benzoyl residue			NULL		0	NULL	NULL	NULL	NULL	NULL	Novel calpain inhibitors derived from phenyl alanine aldehydes or ketoamides carrying a benzoyl residue were prepared and evaluated for their biological potency .	manualset1
81316	1	377405	7	NULL	NULL	0	NULL	Novel chitosan-polycaprolactone 	NonProteinOrNucleicAcidChemical		blends as					potential scaffold	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Novel chitosan-polycaprolactone blends as potential scaffold and carrier for corneal endothelial transplantation .	manualset1
81317	2	377405	7	NULL	NULL	0	NULL	Novel chitosan-polycaprolactone 	NonProteinOrNucleicAcidChemical		carrier for					corneal endothelial transplantation	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Novel chitosan-polycaprolactone blends as potential scaffold and carrier for corneal endothelial transplantation .	manualset1
81318	3	377405	7	NULL	NULL	0	NULL	statement 1	Process		for					corneal endothelial transplantation	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Novel chitosan-polycaprolactone blends as potential scaffold and carrier for corneal endothelial transplantation .	manualset1
81319	1	377406	7	NULL	NULL	0	NULL	Novel combination neo-adjuvant chemotherapy	MedicalProcedure		introduced for					T3 gastric cancer patients	PersonGroup				NULL		0	NULL	NULL	NULL	NULL	NULL	Novel combination neo-adjuvant chemotherapy has been introduced for T3 gastric cancer patients .	manualset1
81320	1	377407	7	NULL	NULL	0	NULL	proximal tubule cell line	Cell	Novel conditionally immortalized human	express					functional influx transporter	GeneOrProtein				NULL		0	NULL	NULL	NULL	NULL	NULL	Novel conditionally immortalized human proximal tubule cell line expressing functional influx and efflux transporters .	manualset1
81321	2	377407	7	NULL	NULL	0	NULL	proximal tubule cell line	Cell	Novel conditionally immortalized human	express					functional efflux transporter	GeneOrProtein				NULL		0	NULL	NULL	NULL	NULL	NULL	Novel conditionally immortalized human proximal tubule cell line expressing functional influx and efflux transporters .	manualset1
81322	1	377408	7	NULL	NULL	NULL	NULL	hnRNP G/RBMX protein	Protein	novel domains in	distinct role in					RNA	NucleicAcidSubstance	binding of			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Novel domains in the hnRNP G/RBMX protein with distinct roles in RNA binding and targeting nascent transcripts .	manualset1
81323	2	377408	7	NULL	NULL	NULL	NULL	hnRNP G/RBMX protein	Protein	novel domains in	distinct role in					nascent transcripts	NucleicAcidSubstance	targeting			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Novel domains in the hnRNP G/RBMX protein with distinct roles in RNA binding and targeting nascent transcripts .	manualset1
81324	1	377410	7	NULL	NULL	0	NULL	nitric oxide synthase	Protein	novel inhibitors of	shows					antioxidant properties	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Novel inhibitors of nitric oxide synthase with antioxidant properties .	manualset1
81325	1	377412	7	NULL	NULL	0	NULL	PKD1 gene	Gene	novel mutations in	occur with					autosomal dominant polycystic kidney disease	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	Novel mutations of PKD1 gene in Chinese patients with autosomal dominant polycystic kidney disease .	manualset1
81326	1	377414	7	NULL	NULL	0	NULL	toluene catabolism	Process	novel pathway of	occur in					bacterium g4	Organism	trichloroethylene-degrading			NULL		0	NULL	NULL	NULL	NULL	NULL	Novel pathway of toluene catabolism in the trichloroethylene-degrading bacterium g4 .	manualset1
81327	1	377416	7	NULL	NULL	0	NULL	Novel polyurethanes	NonProteinOrNucleicAcidChemical		induce					tissue remodeling	Process				NULL	in vivo	0	NULL	NULL	NULL	NULL	NULL	Novel polyurethanes with interconnected porous structure induce in vivo tissue remodeling and accompanied vascularization .	manualset1
81328	2	377416	7	NULL	NULL	0	NULL	Novel polyurethanes	NonProteinOrNucleicAcidChemical		induce					vascularization	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Novel polyurethanes with interconnected porous structure induce in vivo tissue remodeling and accompanied vascularization .	manualset1
81329	3	377416	7	NULL	NULL	0	NULL	Novel polyurethanes	NonProteinOrNucleicAcidChemical		have					 interconnected porous structure	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Novel polyurethanes with interconnected porous structure induce in vivo tissue remodeling and accompanied vascularization .	manualset1
81330	1	377418	7	NULL	NULL	NULL	NULL	serum proteomics	MedicalProcedureOrDevice		predict		may			prostate cancer	Disease	outcome in advanced			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Novel techniques such as serum proteomics , microarrays , and metastatic cell isolation methods may better predict outcome in advanced prostate cancer .	manualset1
81331	2	377418	7	NULL	NULL	0	NULL	microarrays	MedicalProcedureOrDevice		predict		may			prostate cancer	Disease	outcome in advanced			NULL		0	NULL	NULL	NULL	NULL	NULL	Novel techniques such as serum proteomics , microarrays , and metastatic cell isolation methods may better predict outcome in advanced prostate cancer .	manualset1
81332	3	377418	7	NULL	NULL	NULL	NULL	metastatic cell isolation	MedicalProcedureOrDevice		predict		may			prostate cancer	Disease	outcome in advanced			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Novel techniques such as serum proteomics , microarrays , and metastatic cell isolation methods may better predict outcome in advanced prostate cancer .	manualset1
81335	1	377427	7	NULL	NULL	0	NULL	Noxious mechanical stimuli	ExperimentalFactor		increase					iSP	GeneOrProtein	release of			NULL		0	NULL	NULL	NULL	NULL	NULL	Noxious mechanical stimuli , but not thermal stimuli , increased the release of immunoreactive substance P ( iSP ) .	manualset1
81337	2	377427	7	NULL	NULL	0	NULL	thermal stimuli	ExperimentalFactor		does not increase					iSP	GeneOrProtein				NULL		0	NULL	NULL	NULL	NULL	NULL	Noxious mechanical stimuli , but not thermal stimuli , increased the release of immunoreactive substance P ( iSP ) .	manualset1
81340	3	377427	7	NULL	NULL	0	NULL	iSP	GeneOrProtein		is					immunoreactive substance P	GeneOrProtein				NULL		0	NULL	NULL	NULL	NULL	NULL	Noxious mechanical stimuli , but not thermal stimuli , increased the release of immunoreactive substance P ( iSP ) .	manualset1
81343	1	377428	7	NULL	NULL	NULL	NULL	Noxious stimuli	ExperimentalFactor		excite					contralateral topographical projection 	Process	system with 			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Noxious stimuli also excite a system with contralateral topographical projection , high synaptic security and termination in lamina IV .	manualset1
81344	2	377428	7	NULL	NULL	NULL	NULL	Noxious stimuli	ExperimentalFactor		excite					lamina IV	Cell	system with high synaptic security			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Noxious stimuli also excite a system with contralateral topographical projection , high synaptic security and termination in lamina IV .	manualset1
81345	3	377428	7	NULL	NULL	0	NULL	Noxious stimuli	ExperimentalFactor		excite					lamina IV	Cell	termination in			NULL		0	NULL	NULL	NULL	NULL	NULL	Noxious stimuli also excite a system with contralateral topographical projection , high synaptic security and termination in lamina IV .	manualset1
81346	1	377432	7	NULL	NULL	0	NULL	enzymes	Protein		protective against					oxidative stress	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear factor erythroid-derived 2-like 2 ( Nrf2 ) controls the expression of several enzymes that are protective against oxidative stress .	manualset1
81347	2	377432	7	NULL	NULL	0	NULL	Nrf2	Protein		controls					statement 1	Process	expression of			NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear factor erythroid-derived 2-like 2 ( Nrf2 ) controls the expression of several enzymes that are protective against oxidative stress .	manualset1
81348	3	377432	7	NULL	NULL	NULL	NULL	Nrf2	Protein		is					Nuclear factor erythroid-derived 2-like 2	Protein				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nuclear factor erythroid-derived 2-like 2 ( Nrf2 ) controls the expression of several enzymes that are protective against oxidative stress .	manualset1
81349	1	377433	7	NULL	NULL	0	NULL	Nuclear proteins	Protein		isolated from					enterocytes	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear proteins isolated from enterocytes showed increased binding of the HNF-1 alpha complex with a concomitant decrease in the HNF-1 beta-containing complex to the SIF3 element both during the suckling-weaning developmental transition and Caco-2 cell differentiation .	manualset1
81350	2	377433	7	NULL	NULL	0	NULL	HNF-1 alpha complex	Protein		bind					SIF3 element	Gene				NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear proteins isolated from enterocytes showed increased binding of the HNF-1 alpha complex with a concomitant decrease in the HNF-1 beta-containing complex to the SIF3 element both during the suckling-weaning developmental transition and Caco-2 cell differentiation .	manualset1
81351	3	377433	7	NULL	NULL	0	NULL	Nuclear proteins	Protein		increase					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear proteins isolated from enterocytes showed increased binding of the HNF-1 alpha complex with a concomitant decrease in the HNF-1 beta-containing complex to the SIF3 element both during the suckling-weaning developmental transition and Caco-2 cell differentiation .	manualset1
81352	4	377433	7	NULL	NULL	0	NULL	HNF-1 beta-containing complex	Protein		bind					SIF3 element	Gene				NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear proteins isolated from enterocytes showed increased binding of the HNF-1 alpha complex with a concomitant decrease in the HNF-1 beta-containing complex to the SIF3 element both during the suckling-weaning developmental transition and Caco-2 cell differentiation .	manualset1
81353	5	377433	7	NULL	NULL	0	NULL	Nuclear proteins	Protein		decrease					statement 4	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear proteins isolated from enterocytes showed increased binding of the HNF-1 alpha complex with a concomitant decrease in the HNF-1 beta-containing complex to the SIF3 element both during the suckling-weaning developmental transition and Caco-2 cell differentiation .	manualset1
81354	6	377433	7	NULL	NULL	0	NULL	statement 3	Process		during					suckling-weaning developmental transition	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear proteins isolated from enterocytes showed increased binding of the HNF-1 alpha complex with a concomitant decrease in the HNF-1 beta-containing complex to the SIF3 element both during the suckling-weaning developmental transition and Caco-2 cell differentiation .	manualset1
81355	7	377433	7	NULL	NULL	0	NULL	statement 3	Process		during					Caco-2 cell	Cell	differentiation of			NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear proteins isolated from enterocytes showed increased binding of the HNF-1 alpha complex with a concomitant decrease in the HNF-1 beta-containing complex to the SIF3 element both during the suckling-weaning developmental transition and Caco-2 cell differentiation .	manualset1
81356	8	377433	7	NULL	NULL	0	NULL	statement 5	Process		during					suckling-weaning developmental transition	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear proteins isolated from enterocytes showed increased binding of the HNF-1 alpha complex with a concomitant decrease in the HNF-1 beta-containing complex to the SIF3 element both during the suckling-weaning developmental transition and Caco-2 cell differentiation .	manualset1
81357	9	377433	7	NULL	NULL	0	NULL	statement 5	Process		during					Caco-2 cell	Cell	differentiation of			NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear proteins isolated from enterocytes showed increased binding of the HNF-1 alpha complex with a concomitant decrease in the HNF-1 beta-containing complex to the SIF3 element both during the suckling-weaning developmental transition and Caco-2 cell differentiation .	manualset1
81369	1	377434	7	NULL	NULL	0	NULL	Nuclear ribonucleoprotein complexes	Protein		contain					U1 RNA	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear ribonucleoprotein complexes containing U1 and U2 RNA .	manualset1
81374	2	377434	7	NULL	NULL	0	NULL	Nuclear ribonucleoprotein complexes	Protein		contain					U2 RNA	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear ribonucleoprotein complexes containing U1 and U2 RNA .	manualset1
81378	1	377435	7	NULL	NULL	0	NULL	phorbol ester 	NonProteinOrNucleicAcidChemical		induce					interleukin 1 beta	Protein	transcription of			NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear run-on analysis showed that phorbol ester induced the transcription of interleukin 1 beta but did not induce it in the presence of cycloheximide .	manualset1
81381	2	377435	7	NULL	NULL	0	NULL	phorbol ester	NonProteinOrNucleicAcidChemical		does not induce					cycloheximide	NonProteinOrNucleicAcidChemical	in the presence of			NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear run-on analysis showed that phorbol ester induced the transcription of interleukin 1 beta but did not induce it in the presence of cycloheximide .	manualset1
81572	1	377436	7	NULL	NULL	0	NULL	Nuclear tau	Protein		immunoreactivity in					presenile dementia with motor neuron disease	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear tau immunoreactivity in presenile dementia with motor neuron disease : a case report .	manualset1
81573	1	377438	7	NULL	NULL	NULL	NULL	VTs	Protein		stabilize					preproET-1 mRNA transcripts	NucleicAcidSubstance	labile			NULL	endothelial cells	NULL	NULL	NULL	NULL	NULL	NULL	Nuclear transcription and actinomycin D chase experiments indicated that VTs stabilize labile preproET-1 mRNA transcripts in endothelial cells .	manualset1
81574	1	377441	7	NULL	NULL	0	NULL	Nucleoli	CellComponent		is a type of					subnuclear organelles	CellComponent				NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleoli are prominent subnuclear organelles , and are known to be hubs of ribosome synthesis .	manualset1
81575	2	377441	7	NULL	NULL	0	NULL	Nucleoli	CellComponent		hubs of					ribosome synthesis	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleoli are prominent subnuclear organelles , and are known to be hubs of ribosome synthesis .	manualset1
81576	1	377442	7	NULL	NULL	0	NULL	NRTIs	NonProteinOrNucleicAcidChemical		used against					HIV	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleoside reverse transcriptase inhibitors ( NRTIs ) used against the human immunodeficiency virus ( HIV ) need to be activated intracellularly to their triphosphate moiety to inhibit HIV replication .	manualset1
81577	2	377442	7	NULL	NULL	0	NULL	statement 1	Process		activated to					triphosphate moiety	NonProteinOrNucleicAcidChemical	intracellularly			NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleoside reverse transcriptase inhibitors ( NRTIs ) used against the human immunodeficiency virus ( HIV ) need to be activated intracellularly to their triphosphate moiety to inhibit HIV replication .	manualset1
81578	3	377442	7	NULL	NULL	0	NULL	statement 2	Process		inhibit					HIV replication	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleoside reverse transcriptase inhibitors ( NRTIs ) used against the human immunodeficiency virus ( HIV ) need to be activated intracellularly to their triphosphate moiety to inhibit HIV replication .	manualset1
81579	4	377442	7	NULL	NULL	0	NULL	NRTIs	NonProteinOrNucleicAcidChemical		is					Nucleoside reverse transcriptase inhibitors	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleoside reverse transcriptase inhibitors ( NRTIs ) used against the human immunodeficiency virus ( HIV ) need to be activated intracellularly to their triphosphate moiety to inhibit HIV replication .	manualset1
81580	5	377442	7	NULL	NULL	0	NULL	HIV	Organism		is					human immunodeficiency virus	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleoside reverse transcriptase inhibitors ( NRTIs ) used against the human immunodeficiency virus ( HIV ) need to be activated intracellularly to their triphosphate moiety to inhibit HIV replication .	manualset1
81581	1	377443	7	NULL	NULL	NULL	NULL	H2B	Protein	Nucleosomal peptides in histone regions	recognized by			10-33		CD4 T cells	Cell				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nucleosomal peptides in histone regions H2B ( 10-33 ) , H4 ( 16-39 ) ( and overlapping H4 ( 14-28 ) ) , H4 ( 71-94 ) , and H3 ( 91-105 ) ( and overlapping H3 ( 100-114 ) ) were recurrently recognized by CD4 T cells from the patients with lupus .	manualset1
81709	2	377443	7	NULL	NULL	0	NULL	H4	Protein	Nucleosomal peptides in histone regions	recognized by			16-39		CD4 T cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleosomal peptides in histone regions H2B ( 10-33 ) , H4 ( 16-39 ) ( and overlapping H4 ( 14-28 ) ) , H4 ( 71-94 ) , and H3 ( 91-105 ) ( and overlapping H3 ( 100-114 ) ) were recurrently recognized by CD4 T cells from the patients with lupus .	manualset1
81710	3	377443	7	NULL	NULL	0	NULL	overlapping H4	Protein	Nucleosomal peptides in histone regions	recognized by			14-28		CD4 T cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleosomal peptides in histone regions H2B ( 10-33 ) , H4 ( 16-39 ) ( and overlapping H4 ( 14-28 ) ) , H4 ( 71-94 ) , and H3 ( 91-105 ) ( and overlapping H3 ( 100-114 ) ) were recurrently recognized by CD4 T cells from the patients with lupus .	manualset1
81711	4	377443	7	NULL	NULL	0	NULL	H4	Protein	Nucleosomal peptides in histone regions	recognized by			71-94		CD4 T cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleosomal peptides in histone regions H2B ( 10-33 ) , H4 ( 16-39 ) ( and overlapping H4 ( 14-28 ) ) , H4 ( 71-94 ) , and H3 ( 91-105 ) ( and overlapping H3 ( 100-114 ) ) were recurrently recognized by CD4 T cells from the patients with lupus .	manualset1
81712	5	377443	7	NULL	NULL	0	NULL	H3	Protein	Nucleosomal peptides in histone regions	recognized by			91-105		CD4 T cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleosomal peptides in histone regions H2B ( 10-33 ) , H4 ( 16-39 ) ( and overlapping H4 ( 14-28 ) ) , H4 ( 71-94 ) , and H3 ( 91-105 ) ( and overlapping H3 ( 100-114 ) ) were recurrently recognized by CD4 T cells from the patients with lupus .	manualset1
81713	6	377443	7	NULL	NULL	0	NULL	overlapping H3	Protein	Nucleosomal peptides in histone regions	recognized by			100-114		CD4 T cells	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleosomal peptides in histone regions H2B ( 10-33 ) , H4 ( 16-39 ) ( and overlapping H4 ( 14-28 ) ) , H4 ( 71-94 ) , and H3 ( 91-105 ) ( and overlapping H3 ( 100-114 ) ) were recurrently recognized by CD4 T cells from the patients with lupus .	manualset1
81714	7	377443	7	NULL	NULL	0	NULL	statement 1	Process		occur from					lupus	Disease	patients with			NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleosomal peptides in histone regions H2B ( 10-33 ) , H4 ( 16-39 ) ( and overlapping H4 ( 14-28 ) ) , H4 ( 71-94 ) , and H3 ( 91-105 ) ( and overlapping H3 ( 100-114 ) ) were recurrently recognized by CD4 T cells from the patients with lupus .	manualset1
81715	8	377443	7	NULL	NULL	NULL	NULL	statement 2	Process		occur from					lupus	Disease	patients with			NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nucleosomal peptides in histone regions H2B ( 10-33 ) , H4 ( 16-39 ) ( and overlapping H4 ( 14-28 ) ) , H4 ( 71-94 ) , and H3 ( 91-105 ) ( and overlapping H3 ( 100-114 ) ) were recurrently recognized by CD4 T cells from the patients with lupus .	manualset1
81716	9	377443	7	NULL	NULL	0	NULL	statement 3	Process		occur from					lupus	Disease	patients with			NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleosomal peptides in histone regions H2B ( 10-33 ) , H4 ( 16-39 ) ( and overlapping H4 ( 14-28 ) ) , H4 ( 71-94 ) , and H3 ( 91-105 ) ( and overlapping H3 ( 100-114 ) ) were recurrently recognized by CD4 T cells from the patients with lupus .	manualset1
81717	10	377443	7	NULL	NULL	0	NULL	statement 4	Process		occur from					lupus	Disease	patients with			NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleosomal peptides in histone regions H2B ( 10-33 ) , H4 ( 16-39 ) ( and overlapping H4 ( 14-28 ) ) , H4 ( 71-94 ) , and H3 ( 91-105 ) ( and overlapping H3 ( 100-114 ) ) were recurrently recognized by CD4 T cells from the patients with lupus .	manualset1
81718	11	377443	7	NULL	NULL	0	NULL	statement 5	Process		occur from					lupus	Disease	patients with			NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleosomal peptides in histone regions H2B ( 10-33 ) , H4 ( 16-39 ) ( and overlapping H4 ( 14-28 ) ) , H4 ( 71-94 ) , and H3 ( 91-105 ) ( and overlapping H3 ( 100-114 ) ) were recurrently recognized by CD4 T cells from the patients with lupus .	manualset1
81719	12	377443	7	NULL	NULL	0	NULL	statement 6	Process		occur from					lupus	Disease	patients with			NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleosomal peptides in histone regions H2B ( 10-33 ) , H4 ( 16-39 ) ( and overlapping H4 ( 14-28 ) ) , H4 ( 71-94 ) , and H3 ( 91-105 ) ( and overlapping H3 ( 100-114 ) ) were recurrently recognized by CD4 T cells from the patients with lupus .	manualset1
81720	1	377444	7	NULL	NULL	0	NULL	Nucleosome assembly proteins	Protein		important role in					chromatin remodeling	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleosome assembly proteins play important roles in chromatin remodeling , which determines gene expression , cell proliferation and terminal differentiation .	manualset1
81721	2	377444	7	NULL	NULL	NULL	NULL	statement 1	Process		determines					gene expression	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nucleosome assembly proteins play important roles in chromatin remodeling , which determines gene expression , cell proliferation and terminal differentiation .	manualset1
81722	3	377444	7	NULL	NULL	NULL	NULL	statement 1	Process		determines					cell proliferation	Process				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nucleosome assembly proteins play important roles in chromatin remodeling , which determines gene expression , cell proliferation and terminal differentiation .	manualset1
81723	4	377444	7	NULL	NULL	0	NULL	statement 1	Process		determines					terminal differentiation	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleosome assembly proteins play important roles in chromatin remodeling , which determines gene expression , cell proliferation and terminal differentiation .	manualset1
81724	1	377445	7	NULL	NULL	0	NULL	NER	Process	Eukaryotes	involves					multiple gene products	Gene				NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleotide excision repair ( NER ) in eukaryotes is a biochemically complex process involving multiple gene products .	manualset1
81725	2	377445	7	NULL	NULL	0	NULL	NER	Process		is a type of					biochemically complex process	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleotide excision repair ( NER ) in eukaryotes is a biochemically complex process involving multiple gene products .	manualset1
81726	3	377445	7	NULL	NULL	0	NULL	NER	Process		is					Nucleotide excision repair	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleotide excision repair ( NER ) in eukaryotes is a biochemically complex process involving multiple gene products .	manualset1
81727	1	377446	7	NULL	NULL	0	NULL	beta-luffin	Protein		is a type of					ribosome-inactivating protein	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleotide sequence of cDNA encoding beta-luffin , another ribosome-inactivating protein from Luffa cylindrica .	manualset1
81728	2	377446	7	NULL	NULL	0	NULL	beta-luffin	Protein		is obtained from					Luffa cylindrica	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleotide sequence of cDNA encoding beta-luffin , another ribosome-inactivating protein from Luffa cylindrica .	manualset1
81883	1	377448	7	NULL	NULL	0	NULL	CEH-10	GeneOrProtein		regulates					CEH-10	GeneOrProtein	its own expression of			NULL		0	NULL	NULL	NULL	NULL	NULL	Null mutants also fail to express CEH-10 , suggesting that CEH-10 regulates its own expression .	manualset1
81897	1	377455	7	NULL	NULL	0	NULL	GAST-like genes	Gene		identified in					plant species	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous GAST-like genes have been identified in various plant species .	manualset1
81898	1	377457	7	NULL	NULL	NULL	NULL	microglia	Cell	cells with the appearance of 	express		constitutively			class I MHC antigens	Protein				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Numerous cells with the appearance of microglia were found to constitutively express class I MHC antigens , while only rare cells expressed class II ( Ia ) antigens .	manualset1
81899	2	377457	7	NULL	NULL	NULL	NULL	rare cells	Cell		express					class II ( Ia ) antigen	Protein				NULL		NULL	NULL	NULL	NULL	NULL	NULL	Numerous cells with the appearance of microglia were found to constitutively express class I MHC antigens , while only rare cells expressed class II ( Ia ) antigens .	manualset1
81900	1	377458	7	NULL	NULL	0	NULL	neuronal heterotopias	Disease		associated with					ectopic ependymal cavities	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous neuronal heterotopias associated with ectopic ependymal cavities were observed in the vermis in one case .	manualset1
81901	2	377458	7	NULL	NULL	0	NULL	statement 1	Process		occur in					vermis	BodyPart				NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous neuronal heterotopias associated with ectopic ependymal cavities were observed in the vermis in one case .	manualset1
81647	1	387313	11	NULL	NULL	0	NULL	 lesion	MedicalFinding		does not respond to					nafcillin	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The lesion failed to respond to nafcillin alone or combination therapy with hyperbaric oxygen , but showed slow , steady improvement with long-term clindamycin .	manualset1
81648	2	387313	11	NULL	NULL	0	NULL	lesion	MedicalFinding		showed improvement with		 slow;;steady			clindamycin	NonProteinOrNucleicAcidChemical	 long-term			NULL		0	NULL	NULL	NULL	NULL	NULL	The lesion failed to respond to nafcillin alone or combination therapy with hyperbaric oxygen , but showed slow , steady improvement with long-term clindamycin .	manualset1
81649	1	387314	11	NULL	NULL	0	NULL	lesions	MedicalFinding		are					umbilicated	AnatomicalPart	centrally			NULL		0	NULL	NULL	NULL	NULL	NULL	The lesions were centrally umbilicated , resembling molluscum contagiosum , but clearly distinct from Tyson 's glands .	manualset1
81650	2	387314	11	NULL	NULL	0	NULL	 lesions	MedicalFinding		 resemble					molluscum contagiosum	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	The lesions were centrally umbilicated , resembling molluscum contagiosum , but clearly distinct from Tyson 's glands .	manualset1
81651	3	387314	11	NULL	NULL	0	NULL	lesions	MedicalFinding		distinct from		clearly			Tyson 's gland	AnatomicalPart				NULL		0	NULL	NULL	NULL	NULL	NULL	The lesions were centrally umbilicated , resembling molluscum contagiosum , but clearly distinct from Tyson 's glands .	manualset1
81652	1	387315	11	NULL	NULL	0	NULL	 lesions	MedicalFinding		located in					posterolateral thalamus	AnatomicalPart				NULL		0	NULL	NULL	NULL	NULL	NULL	The lesions were located mainly in the posterolateral thalamus including posteromedial part of the internal capsule ( thalamic pain ) , however , they were located outside of the thalamus in some cases ( suprathalamic pain ) .	manualset1
81653	2	387315	11	NULL	NULL	0	NULL	lesions	MedicalFinding		occurs					thalamus	AnatomicalPart	outside			NULL		0	NULL	NULL	NULL	NULL	NULL	The lesions were located mainly in the posterolateral thalamus including posteromedial part of the internal capsule ( thalamic pain ) , however , they were located outside of the thalamus in some cases ( suprathalamic pain ) .	manualset1
81654	3	387315	11	NULL	NULL	0	NULL	statement 1	MedicalFinding		causes					thalamic pain	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	The lesions were located mainly in the posterolateral thalamus including posteromedial part of the internal capsule ( thalamic pain ) , however , they were located outside of the thalamus in some cases ( suprathalamic pain ) .	manualset1
81655	4	387315	11	NULL	NULL	0	NULL	statement 2	MedicalFinding		causes					suprathalamic pain	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	The lesions were located mainly in the posterolateral thalamus including posteromedial part of the internal capsule ( thalamic pain ) , however , they were located outside of the thalamus in some cases ( suprathalamic pain ) .	manualset1
81656	1	387316	11	NULL	NULL	0	NULL	pigs	Organism		infected with					virulent strain	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	The lesions were more strongly expressed in the pigs infected with the virulent strain .	manualset1
81657	2	387316	11	NULL	NULL	0	NULL	lesions	MedicalFinding		expressed in		strongly			statement 1	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	The lesions were more strongly expressed in the pigs infected with the virulent strain .	manualset1
81658	1	387318	11	NULL	NULL	0	NULL	leucocyte migration inhibition	BiologicalProcess		is					LMI	BiologicalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	The leucocyte migration inhibition ( LMI ) was determined in an assay after in vitro challenge with beta-lactoglobulin .	manualset1
81659	1	387319	11	NULL	NULL	0	NULL	leukemia	Disease		is specific to 					strain	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	The leukemia is strain-specific and causes the death of its recipients within 9 days .	manualset1
81660	2	387319	11	NULL	NULL	0	NULL	leukemia	Disease		causes					death	BiologicalProcess	recipient			NULL		0	NULL	NULL	NULL	NULL	NULL	The leukemia is strain-specific and causes the death of its recipients within 9 days .	manualset1
81661	1	387320	11	NULL	NULL	0	NULL	DcCB1 mRNA	NucleicAcidSubstance		is high in					 somatic embryo	Organism part	heart-shaped stage;;globular-shaped stage			NULL		0	NULL	NULL	NULL	NULL	NULL	The level of DcCB1 mRNAs was high in somatic embryos at globular and heart-shaped stages but low in torpedo-shaped somatic embryos .	manualset1
81662	2	387320	11	NULL	NULL	0	NULL	DcCB1 mRNA	NucleicAcidSubstance		is low in					somatic embryo	Organism part	 torpedo-shaped			NULL		0	NULL	NULL	NULL	NULL	NULL	The level of DcCB1 mRNAs was high in somatic embryos at globular and heart-shaped stages but low in torpedo-shaped somatic embryos .	manualset1
81663	1	387321	11	NULL	NULL	NULL	NULL	F antigen	Protein	LNC of MRL/1	increases with		progressively			age	QuantityOrMeasure				NULL		NULL	NULL	NULL	NULL	NULL	NULL	The level of F antigen on LNC of MRL/1 , but not on those of MRL/n mice , increased progressively with age and reached its maximum at 4 mo of age .	manualset1
81667	1	387323	11	NULL	NULL	0	NULL	c-Myc 	Protein		decreased in					ErbB2	Protein	absence of 			NULL		0	NULL	NULL	NULL	NULL	NULL	The level of c-Myc and D-cyclins , proteins involved in p27KiP1 sequestration , decreased in the absence of functional ErbB2 .	manualset1
81668	2	387323	11	NULL	NULL	0	NULL	D-cyclins	Protein		decreased in					ErbB2	Protein	absence of 			NULL		0	NULL	NULL	NULL	NULL	NULL	The level of c-Myc and D-cyclins , proteins involved in p27KiP1 sequestration , decreased in the absence of functional ErbB2 .	manualset1
81669	3	387323	11	NULL	NULL	0	NULL	c-Myc	Protein		involved in					sequestration	BiologicalProcess	p27KiP1			NULL		0	NULL	NULL	NULL	NULL	NULL	The level of c-Myc and D-cyclins , proteins involved in p27KiP1 sequestration , decreased in the absence of functional ErbB2 .	manualset1
81670	4	387323	11	NULL	NULL	0	NULL	D-cyclin	Protein		involved in					sequestration	BiologicalProcess	p27KiP1			NULL		0	NULL	NULL	NULL	NULL	NULL	The level of c-Myc and D-cyclins , proteins involved in p27KiP1 sequestration , decreased in the absence of functional ErbB2 .	manualset1
81671	1	387324	11	NULL	NULL	0	NULL	BMP-2	GeneOrProtein	recombinant;;human	upregulate					connexin43 mRNA	NucleicAcidSubstance				NULL		0	NULL	NULL	NULL	NULL	NULL	The level of connexin43 mRNA is maximally upregulated 48 h after treatment with recombinant human BMP-2 with corresponding changes in protein expression .	manualset1
81672	1	387325	11	NULL	NULL	0	NULL	education													NULL		0	NULL	NULL	NULL	NULL	NULL	The level of education is related to exposure to media as well as the use of family planning methods , and negatively related to the degree of apprehension .	manualset1
81673	1	387326	11	NULL	NULL	0	NULL	infectious pancreatic necrosis virus	Organism		is					IPNV	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	The level of infection by infectious pancreatic necrosis virus ( IPNV ) of kidney macrophages from 12 asymptomatic carrier Atlantic salmon post-smolts was studied .	manualset1
81674	2	387326	11	NULL	NULL	0	NULL	IPNV	Organism		infect					macrophages	Cell	kidney			NULL		0	NULL	NULL	NULL	NULL	NULL	The level of infection by infectious pancreatic necrosis virus ( IPNV ) of kidney macrophages from 12 asymptomatic carrier Atlantic salmon post-smolts was studied .	manualset1
81675	1	387329	11	NULL	NULL	0	NULL	lymphocytes	cell	peritoneal	decreased in					 mice	Organism	Lsp1 ( - / - )			NULL		0	NULL	NULL	NULL	NULL	NULL	The level of peritoneal lymphocytes is decreased in Lsp1 ( - / - ) mice without affecting a particular lymphocytic subset .	manualset1
81676	1	387331	11	NULL	NULL	0	NULL	osteocalcin	Protein		is a marker of					vitamin K2	NonProteinOrNucleicAcidChemical	bone			NULL		0	NULL	NULL	NULL	NULL	NULL	The level of undercarboxylated osteocalcin is recognized as a marker of vitamin K2 bone .	manualset1
81677	1	387334	11	NULL	NULL	NULL	NULL	P450	GeneOrProtein		express					RNA	NucleicAcidSubstance				NULL	fetal hamsters	NULL	NULL	NULL	NULL	NULL	NULL	The levels of RNA expression of both P450s in fetal hamsters were less than 30 % of nonpregnant adult values .	manualset1
81678	1	387338	11	NULL	NULL	0	NULL	ammonium	NonProteinOrNucleicAcidChemical	in cells	reduce the level of					nirB transcript	GeneOrProtein				NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of nirB and ntcB transcripts were low in cells growing on ammonium and increased upon transfer of ammonium-grown cells to nitrate-containing medium .	manualset1
81679	2	387338	11	NULL	NULL	0	NULL	ammonium	NonProteinOrNucleicAcidChemical	in cells	reduce the level of					ntcB transcript	GeneOrProtein				NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of nirB and ntcB transcripts were low in cells growing on ammonium and increased upon transfer of ammonium-grown cells to nitrate-containing medium .	manualset1
81680	3	387338	11	NULL	NULL	0	NULL	nitrate	NonProteinOrNucleicAcidChemical	in cells	increased in the level of					nirB transcript	GeneOrProtein				NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of nirB and ntcB transcripts were low in cells growing on ammonium and increased upon transfer of ammonium-grown cells to nitrate-containing medium .	manualset1
81681	4	387338	11	NULL	NULL	0	NULL	nitrate	NonProteinOrNucleicAcidChemical	in cells	increased in the level of					ntcB transcript\t	GeneOrProtein				NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of nirB and ntcB transcripts were low in cells growing on ammonium and increased upon transfer of ammonium-grown cells to nitrate-containing medium .	manualset1
81682	1	387343	11	NULL	NULL	0	NULL	 lhp1 cyp71	Gene	double mutant	showed					phenotypes	RelationshipPhrase	 severe			NULL		0	NULL	NULL	NULL	NULL	NULL	The lhp1 cyp71 double mutant showed more severe phenotypes than the single mutants , suggesting that AtCYP71 and LHP1 synergistically control plant development .	manualset1
81683	2	387343	11	NULL	NULL	0	NULL	AtCYP71	GeneOrProtein		control 					development	BiologicalProcess	plant			NULL		0	NULL	NULL	NULL	NULL	NULL	The lhp1 cyp71 double mutant showed more severe phenotypes than the single mutants , suggesting that AtCYP71 and LHP1 synergistically control plant development .	manualset1
81684	3	387343	11	NULL	NULL	0	NULL	LHP1	GeneOrProtein		controls					development	BiologicalProcess	plant			NULL		0	NULL	NULL	NULL	NULL	NULL	The lhp1 cyp71 double mutant showed more severe phenotypes than the single mutants , suggesting that AtCYP71 and LHP1 synergistically control plant development .	manualset1
81685	4	387343	11	NULL	NULL	0	NULL	statement 2	Process		is synergistic with					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The lhp1 cyp71 double mutant showed more severe phenotypes than the single mutants , suggesting that AtCYP71 and LHP1 synergistically control plant development .	manualset1
81686	1	387345	11	NULL	NULL	0	NULL	collagenase	GeneOrProtein	fibroblast	has binding site for		putative			 zinc	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The library was screened with an oligonucleotide probe constructed from the putative zinc-binding region of fibroblast collagenase .	manualset1
81687	1	387348	11	NULL	NULL	0	NULL	 ligK gene	Gene		encoding				684-bp open reading frame	polypeptide	PartOfProtein				NULL		0	NULL	NULL	NULL	NULL	NULL	The ligK gene consists of a 684-bp open reading frame encoding a polypeptide with a molecular mass of 24,131 Da .	manualset1
81688	1	387368	11	NULL	NULL	0	NULL	symptomatic epilepsy	Disease	frequency	increased in					elderly population	PersonGroup				NULL		0	NULL	NULL	NULL	NULL	NULL	The literature analysis and our own notices showed that the frequency of symptomatic epilepsy in the elderly population increased .	manualset1
81689	1	387369	11	NULL	NULL	0	NULL	allergic reaction	BiologicalProcess		occurs to					amide 	chemical	local anesthetics			NULL		0	NULL	NULL	NULL	NULL	NULL	The literature demonstrates that an allergic reaction to amide local anesthetics can occur and a thorough history , intradermal testing , and subcutaneous challenge are reasonable approaches to determine a safe agent for subsequent use .	manualset1
81691	1	387378	11	NULL	NULL	0	NULL	 liver	AnatomicalPart		has the capacity to					regenerate	BiologicalProcess	unlimited			NULL		0	NULL	NULL	NULL	NULL	NULL	The liver is an exceptional organ , not only because of its unique anatomical and physiological characteristics , but also because of its unlimited regenerative capacity .	manualset1
81692	1	387380	11	NULL	NULL	0	NULL	transplantation	MedicalProcedureOrDevice	liver 	treats					ATTR amyloidosis	Disease	hereditary			NULL		0	NULL	NULL	NULL	NULL	NULL	The liver transplantation for hereditary ATTR amyloidosis has become a well-established treatment , because the main source of serum variant TTR is shut out .	manualset1
81693	1	387382	11	NULL	NULL	0	NULL	immunoglobulin isotypes			appear in		locally 			 urinary tract	AnatomicalPart	ascending pyelonephritis			NULL		0	NULL	NULL	NULL	NULL	NULL	The local appearance of various immunoglobulin ( Ig ) isotypes in the urinary tract during ascending pyelonephritis was studied in rats experimentally infected with Corynebacterium renale .	manualset1
81694	1	387385	11	NULL	NULL	0	NULL	cobalamin-binding protein	Protein		produces in		locally 			SS	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	The local production of cobalamin-binding proteins in SS was sufficient to achieve concentrations in saliva comparable to the control group .	manualset1
81695	1	387386	11	NULL	NULL	0	NULL	ICP 4	Protein		localized in					infected cells	Cell	herpes simplex virus type 1			NULL		0	NULL	NULL	NULL	NULL	NULL	The localization of ICP 4 , ICP 8 , DNA polymerase and alkaline exonuclease within herpes simplex virus type 1 ( HSV ) - infected cells has been examined by immunofluorescence using specific antibodies to these proteins .	manualset1
81697	1	387392	11	NULL	NULL	0	NULL	GSK3 beta	Protein		hyperphosphorylate					substrate	Protein		 Ser/Thr pentad-repeats		NULL		0	NULL	NULL	NULL	NULL	NULL	The location of this oxyanion binding site in the substrate binding cleft indicates direct coupling of P +4 phosphate-primed substrate binding and catalytic activation , explains the ability of GSK3 beta to processively hyperphosphorylate substrates with Ser/Thr pentad-repeats , and suggests a mechanism for autoinhibition in which the phosphorylated N terminus binds as a competitive pseudosubstrate with phospho-Ser 9 occupying the P +4 site .	manualset1
81698	1	387407	11	NULL	NULL	0	NULL	loss of function	MolecularProcess	 Jhdm2a	results in					obesity	MedicalFinding	mice			NULL		0	NULL	NULL	NULL	NULL	NULL	The loss of Jhdm2a function results in obesity and hyperlipidemia in mice .	manualset1
81699	2	387407	11	NULL	NULL	0	NULL	loss of function	MolecularProcess	 Jhdm2a	results in					hyperlipidemia	MedicalFinding	mice			NULL		0	NULL	NULL	NULL	NULL	NULL	The loss of Jhdm2a function results in obesity and hyperlipidemia in mice .	manualset1
81700	3	387407	11	NULL	NULL	0	NULL	statement 1	Process		occurs along with					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The loss of Jhdm2a function results in obesity and hyperlipidemia in mice .	manualset1
81701	1	387408	11	NULL	NULL	0	NULL	loss of activity	MolecularProcess	PSII	reversed by					Ca ( 2 + )	NonProteinOrNucleicAcidChemical	external medium			NULL		0	NULL	NULL	NULL	NULL	NULL	The loss of PSII activity is reversible by addition of submillimolar amounts of either Ca ( 2 + ) or Na ( + ) to the external medium but not by the addition of any other cation .	manualset1
81702	2	387408	11	NULL	NULL	0	NULL	loss of activity	MolecularProcess	PSII	reversed by					Na ( + )	NonProteinOrNucleicAcidChemical	external medium			NULL		0	NULL	NULL	NULL	NULL	NULL	The loss of PSII activity is reversible by addition of submillimolar amounts of either Ca ( 2 + ) or Na ( + ) to the external medium but not by the addition of any other cation .	manualset1
81703	3	387408	11	NULL	NULL	0	NULL	statement 1	Process		is an alternative to					statement 2	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The loss of PSII activity is reversible by addition of submillimolar amounts of either Ca ( 2 + ) or Na ( + ) to the external medium but not by the addition of any other cation .	manualset1
81704	1	387410	11	NULL	NULL	0	NULL	GAT-1	Protein		is a type of 					GABA transporter	Protein	neuronal			NULL		0	NULL	NULL	NULL	NULL	NULL	The loss of inhibition was accompanied by loss of subclasses of inhibitory interneurons labeled by cholecystokinin and the neuronal GABA transporter GAT-1 , which project axo-somatic and axo-axonic GABAergic inhibitory terminals to granule cells and axon initial segments .	manualset1
81705	2	387410	11	NULL	NULL	0	NULL	GAT-1	Protein		project					 inhibitory terminals	PartOfProtein	axo-somatic;;axo-axonic GABAergic;;granule cells			NULL		0	NULL	NULL	NULL	NULL	NULL	The loss of inhibition was accompanied by loss of subclasses of inhibitory interneurons labeled by cholecystokinin and the neuronal GABA transporter GAT-1 , which project axo-somatic and axo-axonic GABAergic inhibitory terminals to granule cells and axon initial segments .	manualset1
81706	1	387411	11	NULL	NULL	0	NULL	glaucoma	Disease		leads to					loss of sight	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The loss of sight in glaucoma is due to the permanent optic nerve damage which is the result of a chronic elevated intraocular pressure .	manualset1
81707	2	387411	11	NULL	NULL	0	NULL	statement 1	MedicalFinding		is due to					optic nerve damage	MedicalFinding	permanent 			NULL		0	NULL	NULL	NULL	NULL	NULL	The loss of sight in glaucoma is due to the permanent optic nerve damage which is the result of a chronic elevated intraocular pressure .	manualset1
81708	3	387411	11	NULL	NULL	NULL	NULL	intraocular pressure	BiologicalProcess	chronic	damages		permanently 			optic nerve	AnatomicalPart				NULL		NULL	NULL	NULL	NULL	NULL	NULL	The loss of sight in glaucoma is due to the permanent optic nerve damage which is the result of a chronic elevated intraocular pressure .	manualset1
81729	1	387419	11	NULL	NULL	0	NULL	calmodulin	Protein		activates					Ca-ATPase	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	The lower affinity of Met 145-oxidized calmodulin toward the target peptide correlates with experimentally observed lowering of calmodulin-activated Ca-ATPase activity when oxidized calmodulin from aged rat brains is used .	manualset1
81730	1	387420	11	NULL	NULL	0	NULL	PsaK	Protein		is lower in					PSI	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	The lower amount of PsaK present in PSI * may explain its higher electrophoretic mobility .	manualset1
81731	1	387421	11	NULL	NULL	0	NULL	ethylene	NonProteinOrNucleicAcidChemical		is a type of 					hydrocarbon	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The lower hydrocarbons ( ethylene , ethane , and propylene ) were also converted to methane at about 300 degrees C. Conversion of benzene was also possible when other hydrocarbons were present at high concentrations .	manualset1
81732	2	387421	11	NULL	NULL	0	NULL	 ethane	NonProteinOrNucleicAcidChemical		is a type of 					hydrocarbon	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The lower hydrocarbons ( ethylene , ethane , and propylene ) were also converted to methane at about 300 degrees C. Conversion of benzene was also possible when other hydrocarbons were present at high concentrations .	manualset1
81733	3	387421	11	NULL	NULL	0	NULL	propylene	NonProteinOrNucleicAcidChemical		is a type of 					hydrocarbon	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The lower hydrocarbons ( ethylene , ethane , and propylene ) were also converted to methane at about 300 degrees C. Conversion of benzene was also possible when other hydrocarbons were present at high concentrations .	manualset1
81734	4	387421	11	NULL	NULL	0	NULL	ethylene	NonProteinOrNucleicAcidChemical		is converted to					methane	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The lower hydrocarbons ( ethylene , ethane , and propylene ) were also converted to methane at about 300 degrees C. Conversion of benzene was also possible when other hydrocarbons were present at high concentrations .	manualset1
81735	5	387421	11	NULL	NULL	0	NULL	ethane	NonProteinOrNucleicAcidChemical		is converted to					methane	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The lower hydrocarbons ( ethylene , ethane , and propylene ) were also converted to methane at about 300 degrees C. Conversion of benzene was also possible when other hydrocarbons were present at high concentrations .	manualset1
81736	6	387421	11	NULL	NULL	0	NULL	propylene	NonProteinOrNucleicAcidChemical		is converted to					methane	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The lower hydrocarbons ( ethylene , ethane , and propylene ) were also converted to methane at about 300 degrees C. Conversion of benzene was also possible when other hydrocarbons were present at high concentrations .	manualset1
81737	7	387421	11	NULL	NULL	0	NULL	benzene	NonProteinOrNucleicAcidChemical		is converted to					methane	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The lower hydrocarbons ( ethylene , ethane , and propylene ) were also converted to methane at about 300 degrees C. Conversion of benzene was also possible when other hydrocarbons were present at high concentrations .	manualset1
81738	1	387425	11	NULL	NULL	0	NULL	angiotensin II 	Protein	low	has no effect on					water intake	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The lowest doses of angiotensin II ( 25 and 50 micrograms/kg SC ) had no significant effect on either water intake or urine output .	manualset1
81739	2	387425	11	NULL	NULL	0	NULL	angiotensin II	Protein	low	has no effect on					urine output	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The lowest doses of angiotensin II ( 25 and 50 micrograms/kg SC ) had no significant effect on either water intake or urine output .	manualset1
81740	1	387428	11	NULL	NULL	0	NULL	 lubricants	Chemical		are based on					 mineral hydrocarbon	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The lubricants were based on mineral hydrocarbon fractions .	manualset1
81741	1	387434	11	NULL	NULL	0	NULL	lung ball	MedicalFinding		is a type of 					pulmonary aspergillosis	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	The lung ball is a special type of pulmonary aspergillosis ( PA ) occurring often after chemotherapy for leukemia .	manualset1
81742	2	387434	11	NULL	NULL	0	NULL	pulmonary aspergillosis	Disease		is					PA	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	The lung ball is a special type of pulmonary aspergillosis ( PA ) occurring often after chemotherapy for leukemia .	manualset1
81743	3	387434	11	NULL	NULL	0	NULL	pulmonary aspergillosis	Disease		occurs after					leukemia	Disease	chemotherapy for			NULL		0	NULL	NULL	NULL	NULL	NULL	The lung ball is a special type of pulmonary aspergillosis ( PA ) occurring often after chemotherapy for leukemia .	manualset1
81744	1	387437	11	NULL	NULL	0	NULL	acidic forms	Organism	lung	eliminated by					neuraminidase	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	The lung preparation also contained more acidic forms ( pI = 4 -- 5 ) , which were eliminated by treatment with neuraminidase .	manualset1
81745	1	387438	11	NULL	NULL	0	NULL	oxymetholone	NonProteinOrNucleicAcidChemical		has					luteolytic activity	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The luteolytic activity of oxymetholone , and anabolic steroid , has been evaluated in 10 women .	manualset1
81746	1	387447	11	NULL	NULL	0	NULL	macrogamonts	cell		have a					nucleus	CellComponent	large			NULL		0	NULL	NULL	NULL	NULL	NULL	The macrogamonts develop below the nucleus of the host cell and have a large nucleus with a prominent nucleolus .	manualset1
81747	1	387453	11	NULL	NULL	0	NULL	magnetic urokinase	Protein		has 					fibrinolytic activity	BiologicalProcess	high			NULL		0	NULL	NULL	NULL	NULL	NULL	The magnetic urokinase dispersed in saline and exerted high fibrinolytic activity ( 13.8 X 10 ( 4 ) IU/mg protein ) , and was readily recovered from saline by magnetic force of 250 Oe .	manualset1
81748	1	387460	11	NULL	NULL	0	NULL	yohimbine	NonProteinOrNucleicAcidChemical		induces					reinstatement	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of yohimbine-induced reinstatement was similar regardless of the presence or absence of the cocaine-paired stimulus .	manualset1
81750	1	387475	11	NULL	NULL	0	NULL	staphylococcus	Organism		causes					sepsis	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The main pathogene of sepsis at present is staphylococcus .	manualset1
81751	1	387479	11	NULL	NULL	0	NULL	anastomotic construction	MedicalFinding	colon;;rectum	include					dehiscence	BiologicalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	The main serious risks of anastomotic construction in the colon and rectum include dehiscence and stricture formation .	manualset1
81752	2	387479	11	NULL	NULL	0	NULL	anastomotic construction	MedicalFinding	colon;;rectum\t	include					stricture formation	BiologicalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	The main serious risks of anastomotic construction in the colon and rectum include dehiscence and stricture formation .	manualset1
81753	1	387483	11	NULL	NULL	0	NULL	maize	Organism		is a synonym of					Zea mays	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	The maize ( Zea mays ) genome appears to contain at least 17 different CycD genes , and they fall into the subgroups previously described for other plants .	manualset1
81754	2	387483	11	NULL	NULL	0	NULL	maize	Organism		contain					CycD gene	Gene				NULL		0	NULL	NULL	NULL	NULL	NULL	The maize ( Zea mays ) genome appears to contain at least 17 different CycD genes , and they fall into the subgroups previously described for other plants .	manualset1
81755	1	387486	11	NULL	NULL	0	NULL	ampullate gland	AnatomicalPart	major	is present in					Latrodectus hesperus	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	The major ampullate gland of Latrodectus hesperus ( black widow ) is similar in morphology to those found in the Araneid spiders .	manualset1
81756	2	387486	11	NULL	NULL	0	NULL	ampullate gland	AnatomicalPart	Latrodectus hesperus	similar to		morphological 			ampullate gland	AnatomicalPart	Araneid spider			NULL		0	NULL	NULL	NULL	NULL	NULL	The major ampullate gland of Latrodectus hesperus ( black widow ) is similar in morphology to those found in the Araneid spiders .	manualset1
81757	1	387487	11	NULL	NULL	0	NULL	carbonyl reduction	MolecularProcess		is a part of 					 biotransformation	BiologicalProcess	major			NULL		0	NULL	NULL	NULL	NULL	NULL	The major biotransformation pathways are carbonyl reduction , O-methylation at C-3 ' , O-methylation after aromatic hydroxylation at the position C-2 ' on phenyl B ring and O-demethylation on A ring .	manualset1
81758	2	387487	11	NULL	NULL	0	NULL	O-methylation	MolecularProcess		is a part of 				C-3 '	biotransformation	BiologicalProcess	major			NULL		0	NULL	NULL	NULL	NULL	NULL	The major biotransformation pathways are carbonyl reduction , O-methylation at C-3 ' , O-methylation after aromatic hydroxylation at the position C-2 ' on phenyl B ring and O-demethylation on A ring .	manualset1
81759	3	387487	11	NULL	NULL	0	NULL	 phenyl B ring	Chemical	C-2 '	undergoes					hydroxylation	MolecularProcess	aromatic			NULL		0	NULL	NULL	NULL	NULL	NULL	The major biotransformation pathways are carbonyl reduction , O-methylation at C-3 ' , O-methylation after aromatic hydroxylation at the position C-2 ' on phenyl B ring and O-demethylation on A ring .	manualset1
81760	4	387487	11	NULL	NULL	0	NULL	statement 3	Chemical		undergoes					O-methylation	MolecularProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	The major biotransformation pathways are carbonyl reduction , O-methylation at C-3 ' , O-methylation after aromatic hydroxylation at the position C-2 ' on phenyl B ring and O-demethylation on A ring .	manualset1
81761	5	387487	11	NULL	NULL	0	NULL	statement 4	Process		occurs after					statement 3	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The major biotransformation pathways are carbonyl reduction , O-methylation at C-3 ' , O-methylation after aromatic hydroxylation at the position C-2 ' on phenyl B ring and O-demethylation on A ring .	manualset1
81762	6	387487	11	NULL	NULL	0	NULL	A ring	Chemical		undergoes					O-demethylation 	MolecularProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	The major biotransformation pathways are carbonyl reduction , O-methylation at C-3 ' , O-methylation after aromatic hydroxylation at the position C-2 ' on phenyl B ring and O-demethylation on A ring .	manualset1
81763	7	387487	11	NULL	NULL	0	NULL	statement 4	Process		is a part of 					biotransformation	BiologicalProcess	major			NULL		0	NULL	NULL	NULL	NULL	NULL	The major biotransformation pathways are carbonyl reduction , O-methylation at C-3 ' , O-methylation after aromatic hydroxylation at the position C-2 ' on phenyl B ring and O-demethylation on A ring .	manualset1
81764	8	387487	11	NULL	NULL	0	NULL	statement 6	Process		is a part of 					biotransformation	BiologicalProcess	major			NULL		0	NULL	NULL	NULL	NULL	NULL	The major biotransformation pathways are carbonyl reduction , O-methylation at C-3 ' , O-methylation after aromatic hydroxylation at the position C-2 ' on phenyl B ring and O-demethylation on A ring .	manualset1
81765	1	387488	11	NULL	NULL	NULL	NULL	death	BiologicalProcess	hemophiliacs	is related to		cause			bleeding	BiologicalProcess				NULL		NULL	NULL	NULL	NULL	NULL	NULL	The major causes of death not related to AIDS in hemophiliacs were bleeding , liver cirrhosis , and liver cancer .	manualset1
81766	2	387488	11	NULL	NULL	NULL	NULL	death	BiologicalProcess	hemophiliacs	is related to		cause			liver cirrhosis	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	The major causes of death not related to AIDS in hemophiliacs were bleeding , liver cirrhosis , and liver cancer .	manualset1
81767	3	387488	11	NULL	NULL	NULL	NULL	death	BiologicalProcess	hemophiliacs	is related to		cause			liver cancer	MedicalFinding				NULL		NULL	NULL	NULL	NULL	NULL	NULL	The major causes of death not related to AIDS in hemophiliacs were bleeding , liver cirrhosis , and liver cancer .	manualset1
81768	4	387488	11	NULL	NULL	0	NULL	death	BiologicalProcess	hemophiliacs	is not related to		cause			AIDS	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The major causes of death not related to AIDS in hemophiliacs were bleeding , liver cirrhosis , and liver cancer .	manualset1
81769	1	387489	11	NULL	NULL	0	NULL	atrial natriuretic peptide	GeneOrProtein		is					ANP	GeneOrProtein				NULL		0	NULL	NULL	NULL	NULL	NULL	The major class of atrial natriuretic peptide ( ANP ) receptors was isolated from cultured vascular smooth muscle cells , and a partial amino acid sequence was obtained .	manualset1
81770	2	387489	11	NULL	NULL	0	NULL	atrial natriuretic peptide receptor	GeneOrProtein		is isolated from					vascular smooth muscle cell	Cell	cultured			NULL		0	NULL	NULL	NULL	NULL	NULL	The major class of atrial natriuretic peptide ( ANP ) receptors was isolated from cultured vascular smooth muscle cells , and a partial amino acid sequence was obtained .	manualset1
81771	1	387490	11	NULL	NULL	NULL	NULL	rose water	Chemical		obtained from					bud	AnatomicalPart	cultivar Ranisahiba 			NULL		NULL	NULL	NULL	NULL	NULL	NULL	The major components of rose water volatiles obtained from the bud , half bloom and full bloom stages of cultivar ` Ranisahiba ' were phenyl ethyl alcohol ( 66.2-79 .0 % ) , geraniol ( 3.3-6 .6 % ) and citronellol ( 1.8-5 .5 % ) .	manualset1
81772	2	387490	11	NULL	NULL	NULL	NULL	rose water	Chemical		obtained from					 half bloom	AnatomicalPart	cultivar Ranisahiba			NULL		NULL	NULL	NULL	NULL	NULL	NULL	The major components of rose water volatiles obtained from the bud , half bloom and full bloom stages of cultivar ` Ranisahiba ' were phenyl ethyl alcohol ( 66.2-79 .0 % ) , geraniol ( 3.3-6 .6 % ) and citronellol ( 1.8-5 .5 % ) .	manualset1
81773	3	387490	11	NULL	NULL	NULL	NULL	rose water	Chemical		obtained from					full bloom	AnatomicalPart	cultivar Ranisahiba			NULL		NULL	NULL	NULL	NULL	NULL	NULL	The major components of rose water volatiles obtained from the bud , half bloom and full bloom stages of cultivar ` Ranisahiba ' were phenyl ethyl alcohol ( 66.2-79 .0 % ) , geraniol ( 3.3-6 .6 % ) and citronellol ( 1.8-5 .5 % ) .	manualset1
81774	4	387490	11	NULL	NULL	0	NULL	rose water	Chemical	volatiles of	composed of 					phenyl ethyl alcohol	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The major components of rose water volatiles obtained from the bud , half bloom and full bloom stages of cultivar ` Ranisahiba ' were phenyl ethyl alcohol ( 66.2-79 .0 % ) , geraniol ( 3.3-6 .6 % ) and citronellol ( 1.8-5 .5 % ) .	manualset1
81775	5	387490	11	NULL	NULL	0	NULL	rose water	Chemical	volatiles of	composed of 					geraniol	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The major components of rose water volatiles obtained from the bud , half bloom and full bloom stages of cultivar ` Ranisahiba ' were phenyl ethyl alcohol ( 66.2-79 .0 % ) , geraniol ( 3.3-6 .6 % ) and citronellol ( 1.8-5 .5 % ) .	manualset1
81776	6	387490	11	NULL	NULL	0	NULL	rose water	Chemical	volatiles of	composed of 					citronellol 	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The major components of rose water volatiles obtained from the bud , half bloom and full bloom stages of cultivar ` Ranisahiba ' were phenyl ethyl alcohol ( 66.2-79 .0 % ) , geraniol ( 3.3-6 .6 % ) and citronellol ( 1.8-5 .5 % ) .	manualset1
81777	1	387492	11	NULL	NULL	0	NULL	triathlon	Process		contains					running stage	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The major decrease in plasma volume was during the running stage of the triathlon during which it decreased by 6.2 % + / - 1.7 % , of which 3.0 % + / - 1.8 % was attributable to exercise alone .	manualset1
81778	2	387492	11	NULL	NULL	0	NULL	statement 1	Process		reduces					volume	Quantity	plasma			NULL		0	NULL	NULL	NULL	NULL	NULL	The major decrease in plasma volume was during the running stage of the triathlon during which it decreased by 6.2 % + / - 1.7 % , of which 3.0 % + / - 1.8 % was attributable to exercise alone .	manualset1
81779	1	387494	11	NULL	NULL	0	NULL	silty sediment 	EnvironmentalFactor		is rich in					omega-3 PUFAs	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The major difference in the fatty acid composition of M. plumulosa cultured on silty sediment compared to amphipods cultured on a sand substrate and both fed Sera micron was an increase in the ratio of omega-3 to omega-6 PUFAs , indicating that the silty sediment provides additional food sources rich in omega-3 PUFAs .	manualset1
81780	1	387495	11	NULL	NULL	0	NULL	transplantation immunology	MedicalProcedureOrDevice		aims on					allograft transplants	AnatomicalPart	tolerance to			NULL		0	NULL	NULL	NULL	NULL	NULL	The major goal of transplantation immunology is to develop tolerance to allograft transplants and long-term drug-free survival .	manualset1
81781	2	387495	11	NULL	NULL	0	NULL	transplantation immunology	MedicalProcedureOrDevice		aims on					drug-free survival	BiologicalProcess	long-term			NULL		0	NULL	NULL	NULL	NULL	NULL	The major goal of transplantation immunology is to develop tolerance to allograft transplants and long-term drug-free survival .	manualset1
81782	1	387496	11	NULL	NULL	0	NULL	trauma	MedicalFinding		is an indication for					amputation	MedicalFinding	upper limb			NULL		0	NULL	NULL	NULL	NULL	NULL	The major indication for upper limb amputation was trauma and post-fracture splintage gangrene ( 57 % ) .	manualset1
81783	2	387496	11	NULL	NULL	0	NULL	splintage gangrene	MedicalFinding	post-fracture	is an indication for					amputation	MedicalFinding	upper limb			NULL		0	NULL	NULL	NULL	NULL	NULL	The major indication for upper limb amputation was trauma and post-fracture splintage gangrene ( 57 % ) .	manualset1
81785	1	387504	11	NULL	NULL	0	NULL	 emphysema	MedicalFinding		is a type of 					lung disease	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	The major underlying lung diseases associated with SSP were emphysema ( 22 patients ) and tuberculosis ( 21 patients ) .	manualset1
81786	2	387504	11	NULL	NULL	0	NULL	tuberculosis	MedicalFinding		is a type of 					lung disease	Disease				NULL		0	NULL	NULL	NULL	NULL	NULL	The major underlying lung diseases associated with SSP were emphysema ( 22 patients ) and tuberculosis ( 21 patients ) .	manualset1
81787	3	387504	11	NULL	NULL	0	NULL	emphysema 	MedicalFinding		is associated with					SSP	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The major underlying lung diseases associated with SSP were emphysema ( 22 patients ) and tuberculosis ( 21 patients ) .	manualset1
81788	4	387504	11	NULL	NULL	0	NULL	tuberculosis	MedicalFinding		is associated with					SSP	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The major underlying lung diseases associated with SSP were emphysema ( 22 patients ) and tuberculosis ( 21 patients ) .	manualset1
81789	1	387506	11	NULL	NULL	0	NULL	compounds	Chemical		transport					membrane	CellComponent	across			NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of ABC domains energize the transport of compounds across the membranes .	manualset1
81790	2	387506	11	NULL	NULL	0	NULL	ABC domain	PartOfProtein		energize					statement 1	Process				NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of ABC domains energize the transport of compounds across the membranes .	manualset1
81791	1	387507	11	NULL	NULL	0	NULL	IC neurons	cell		increases					action potential	Process	current-evoked			NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of IC neurons ( 66 % ) displayed an increase in current-evoked action potentials ( Positive Gain ) .	manualset1
81792	1	387508	11	NULL	NULL	0	NULL	human gene	Gene	majority	are conserved among					mammals	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of human genes are conserved among mammals , but some gene families have undergone extensive expansion in particular lineages .	manualset1
81793	1	387509	11	NULL	NULL	0	NULL	squamous cell carcinoma	MedicalFinding	majority	is a type of 					tumor	MedicalFinding	induced			NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of induced tumors were squamous cell carcinomas .	manualset1
81794	1	387515	11	NULL	NULL	0	NULL	ANAE	Protein		are active in					membrane	CellComponent	lymphocytes			NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the ANAE activity in lymphocytes was found to be membrane bound .	manualset1
81795	1	387516	11	NULL	NULL	NULL	NULL	Golgi tendon organ	AnatomicalPart	majority of	does not produce					discharge	Chemical	spontaneous			NULL		NULL	NULL	NULL	NULL	NULL	NULL	The majority of the Golgi tendon organs , pressure receptors , and the elementary dynamic and static receptors of the muscle spindles did not produce spontaneous discharges .	manualset1
81796	2	387516	11	NULL	NULL	NULL	NULL	pressure receptor	AnatomicalPart	majority	does not produce					discharge	Chemical	spontaneous			NULL		NULL	NULL	NULL	NULL	NULL	NULL	The majority of the Golgi tendon organs , pressure receptors , and the elementary dynamic and static receptors of the muscle spindles did not produce spontaneous discharges .	manualset1
81797	3	387516	11	NULL	NULL	NULL	NULL	dynamic receptor	AnatomicalPart	muscle spindles	does not produce					discharge	Chemical	spontaneous			NULL		NULL	NULL	NULL	NULL	NULL	NULL	The majority of the Golgi tendon organs , pressure receptors , and the elementary dynamic and static receptors of the muscle spindles did not produce spontaneous discharges .	manualset1
81798	4	387516	11	NULL	NULL	NULL	NULL	static receptor	AnatomicalPart	muscle spindles	does not produce					discharge	Chemical	spontaneous			NULL		NULL	NULL	NULL	NULL	NULL	NULL	The majority of the Golgi tendon organs , pressure receptors , and the elementary dynamic and static receptors of the muscle spindles did not produce spontaneous discharges .	manualset1
81799	1	387518	11	NULL	NULL	0	NULL	Bacillus	Organism		is a type of 					bacteria	Organism	airborne			NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the airborne bacteria belonged to the genera Bacillus , Micrococcus , and Staphylococcus , but a total of 37 different genera were identified in the air .	manualset1
81800	2	387518	11	NULL	NULL	0	NULL	Micrococcus	Organism		is a type of 					bacteria	Organism	airborne			NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the airborne bacteria belonged to the genera Bacillus , Micrococcus , and Staphylococcus , but a total of 37 different genera were identified in the air .	manualset1
81801	3	387518	11	NULL	NULL	0	NULL	Staphylococcus	Organism		is a type of 					bacteria	Organism	airborne			NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the airborne bacteria belonged to the genera Bacillus , Micrococcus , and Staphylococcus , but a total of 37 different genera were identified in the air .	manualset1
81802	1	387524	11	NULL	NULL	0	NULL	gastric ulcer	MedicalFinding	coexisting	occurres in					pyloric gland area	AnatomicalPart	antrofundic border			NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of these coexisting gastric ulcers occurred in the pyloric gland area adjacent to the antrofundic border , and all the duodenal ulcers in the proximal duodenum .	manualset1
81803	2	387524	11	NULL	NULL	0	NULL	duodenal ulcers	MedicalFinding		occurred in					duodenum	AnatomicalPart	proximal 			NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of these coexisting gastric ulcers occurred in the pyloric gland area adjacent to the antrofundic border , and all the duodenal ulcers in the proximal duodenum .	manualset1
81804	1	387525	11	NULL	NULL	0	NULL	teratomas	MedicalFinding	majority	are					solid	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of these teratomas are solid or mixed cystic and solid external caudal masses .	manualset1
81805	2	387525	11	NULL	NULL	0	NULL	teratomas	MedicalFinding	majority of	are					cystic	MedicalFinding	mixed			NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of these teratomas are solid or mixed cystic and solid external caudal masses .	manualset1
81806	3	387525	11	NULL	NULL	0	NULL	statement 1	MedicalFinding		is an alternative to					statement 2	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of these teratomas are solid or mixed cystic and solid external caudal masses .	manualset1
81807	4	387525	11	NULL	NULL	0	NULL	teratomas	MedicalFinding	majority of	have					solid caudal mass	AnatomicalPart	external 			NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of these teratomas are solid or mixed cystic and solid external caudal masses .	manualset1
81808	1	387528	11	NULL	NULL	0	NULL	deformities	MedicalFinding	vertebral 	are					asymptomatic	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of vertebral deformities are asymptomatic and thus definition is normally based on radiographic appearance .	manualset1
81810	1	387532	11	NULL	NULL	0	NULL	lethality	BiologicalProcess	male	is suppressed by					mutations	MolecularProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	The male lethality is suppressed by mutations that force all animals into the XO mode of both processes .	manualset1
81811	1	387535	11	NULL	NULL	0	NULL	malignant cells	cell		can avoid initiation of 					Mvarphi	Cell				NULL		0	NULL	NULL	NULL	NULL	NULL	The malignant cells can thereby avoid initiation of potentially dangerous Mvarphi functions and create favorable conditions for tumor progression .	manualset1
81814	2	387535	11	NULL	NULL	0	NULL	statement 1	Process		is favorable for					tumor progression	BiologicalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	The malignant cells can thereby avoid initiation of potentially dangerous Mvarphi functions and create favorable conditions for tumor progression .	manualset1
81816	1	387541	11	NULL	NULL	0	NULL	bone graft	MedicalProcedureOrDevice	iliac crest	widened					manubrium	AnatomicalPart				NULL		0	NULL	NULL	NULL	NULL	NULL	The manubrium was widened using an iliac crest bone graft , stabilised using internal fixation plates and reconstructed with a pectoral muscle flap .	manualset1
81850	1	387544	11	NULL	NULL	0	NULL	Dysidea avara	Organism		is a type of					marine sponge	Organism				NULL		0	NULL	NULL	NULL	NULL	NULL	The marine sponge Dysidea avara contained avarol ( 1 ) and avarone ( 2 ) .	manualset1
81851	2	387544	11	NULL	NULL	0	NULL	Dysidea avara	Organism		contains					avarol	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The marine sponge Dysidea avara contained avarol ( 1 ) and avarone ( 2 ) .	manualset1
81852	3	387544	11	NULL	NULL	0	NULL	Dysidea avara	Organism		contains					avarone	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The marine sponge Dysidea avara contained avarol ( 1 ) and avarone ( 2 ) .	manualset1
81853	1	387549	11	NULL	NULL	0	NULL	lymphocytic choriomeningitis virus	Organism		causes					massive inflammation	MedicalFinding	cerebrospinal fluid;;adult mice			NULL		0	NULL	NULL	NULL	NULL	NULL	The massive inflammation of the cerebrospinal fluid ( CSF ) which occurs in adult mice injected with lymphocytic choriomeningitis virus ( LCMV ) has been analyzed by flow microfluorometry ( FMF ) .	manualset1
81854	1	387552	11	NULL	NULL	0	NULL	humerus 	AnatomicalPart		has more strength than		material			tibiotarsus	AnatomicalPart				NULL		0	NULL	NULL	NULL	NULL	NULL	The material strength of the humerus was greater than the tibiotarsus ; this difference in strength was reflected in both the collagen and mineral matrix biochemistry .	manualset1
81855	1	387554	11	NULL	NULL	0	NULL	 immune response	BiologicalProcess	maternal	effects					 platelet GPIb	CellComponent	fetal			NULL		0	NULL	NULL	NULL	NULL	NULL	The maternal immune response to fetal platelet GPIb causes frequent miscarriage in mice that can be prevented by intravenous IgG and anti-FcRn therapies .	manualset1
81856	2	387554	11	NULL	NULL	0	NULL	statement 1	process		causes					miscarriage	BiologicalProcess	 mice			NULL		0	NULL	NULL	NULL	NULL	NULL	The maternal immune response to fetal platelet GPIb causes frequent miscarriage in mice that can be prevented by intravenous IgG and anti-FcRn therapies .	manualset1
81857	3	387554	11	NULL	NULL	0	NULL	IgG	Protein	intravenous	treats					miscarriage	BiologicalProcess	mice			NULL		0	NULL	NULL	NULL	NULL	NULL	The maternal immune response to fetal platelet GPIb causes frequent miscarriage in mice that can be prevented by intravenous IgG and anti-FcRn therapies .	manualset1
81858	1	387559	11	NULL	NULL	0	NULL	VSV G protein	Protein	wild-type;;mature	is a					trimer	Protein	noncovalently associated			NULL		0	NULL	NULL	NULL	NULL	NULL	The mature wild-type VSV G protein is a noncovalently associated trimer .	manualset1
81859	1	387560	11	NULL	NULL	0	NULL	mau gene cluster	Gene		encode 					mauJ product	PartOfProtein	polypeptide			NULL		0	NULL	NULL	NULL	NULL	NULL	The mauJ product is the only polypeptide encoded by the mau gene cluster which is predicted to be cytoplasmic .	manualset1
81860	1	387561	11	NULL	NULL	0	NULL	maxillary tuberosity region	AnatomicalPart		is involved in					preprosthetic surgery	MedicalProcedureOrDevice				NULL		0	NULL	NULL	NULL	NULL	NULL	The maxillary tuberosity region is becoming increasingly involved in preprosthetic surgery as part of a comprehensive implant treatment planning .	manualset1
81861	1	387595	11	NULL	NULL	0	NULL	 Maalox 	NonProteinOrNucleicAcidChemical		produces 					bilesalt	chemical	less			NULL		0	NULL	NULL	NULL	NULL	NULL	The mean bile salt concentration of those treated with Maalox ( 0.24 mM ) , Meciadanol ( 0.24 mM ) , or sucralfate ( 0.35 mM ) was significantly lower than those treated with nasogastric aspiration ( 0.87 mM ) alone ( P less than 0.01 ) .	manualset1
81862	2	387595	11	NULL	NULL	0	NULL	Meciadanol	NonProteinOrNucleicAcidChemical		produces					bilesalt	chemical	less			NULL		0	NULL	NULL	NULL	NULL	NULL	The mean bile salt concentration of those treated with Maalox ( 0.24 mM ) , Meciadanol ( 0.24 mM ) , or sucralfate ( 0.35 mM ) was significantly lower than those treated with nasogastric aspiration ( 0.87 mM ) alone ( P less than 0.01 ) .	manualset1
81863	3	387595	11	NULL	NULL	0	NULL	sucralfate	NonProteinOrNucleicAcidChemical		produces					bilesalt	chemical	less			NULL		0	NULL	NULL	NULL	NULL	NULL	The mean bile salt concentration of those treated with Maalox ( 0.24 mM ) , Meciadanol ( 0.24 mM ) , or sucralfate ( 0.35 mM ) was significantly lower than those treated with nasogastric aspiration ( 0.87 mM ) alone ( P less than 0.01 ) .	manualset1
81864	4	387595	11	NULL	NULL	0	NULL	nasogastric aspiration	AnatomicalPart		produces					bilesalt	chemical	more			NULL		0	NULL	NULL	NULL	NULL	NULL	The mean bile salt concentration of those treated with Maalox ( 0.24 mM ) , Meciadanol ( 0.24 mM ) , or sucralfate ( 0.35 mM ) was significantly lower than those treated with nasogastric aspiration ( 0.87 mM ) alone ( P less than 0.01 ) .	manualset1
81865	1	387611	11	NULL	NULL	0	NULL	FSH	chemical	high	higher the severity of					liver cirrhosis	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The mean percentage increase of FSH and LH was higher the greater the severity of liver cirrhosis .	manualset1
81866	2	387611	11	NULL	NULL	0	NULL	LH	chemical	high	higher the severity of					liver cirrhosis	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The mean percentage increase of FSH and LH was higher the greater the severity of liver cirrhosis .	manualset1
81867	1	387620	11	NULL	NULL	0	NULL	 infection	MedicalFinding	central nervous system	onsets 					epilepsy	MedicalFinding				NULL		0	NULL	NULL	NULL	NULL	NULL	The mean time of onset of epilepsy after central nervous system infection was 1.4 + / - 0.9 years ( range 0-19 years ) .	manualset1
81868	1	387626	11	NULL	NULL	0	NULL	measles-mumps-rubella vaccine 	MedicalProcedureOrDevice		has					biosafety	BiologicalProcess	high			NULL		0	NULL	NULL	NULL	NULL	NULL	The measles-mumps-rubella ( MMR ) vaccine has been very effective in the elimination of disease and has high biosafety .	manualset1
81869	2	387626	11	NULL	NULL	0	NULL	measles-mumps-rubella	MedicalProcedureOrDevice		is					MMR	MedicalProcedureOrDevice				NULL		0	NULL	NULL	NULL	NULL	NULL	The measles-mumps-rubella ( MMR ) vaccine has been very effective in the elimination of disease and has high biosafety .	manualset1
81870	1	387641	11	NULL	NULL	0	NULL	phosphate	NonProteinOrNucleicAcidChemical	intestine	transports via					proton symporter	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism of the transport of phosphate in the intestine is via a proton symporter whilst in the parotid gland it is effected by a Na + coupled transporter .	manualset1
81871	2	387641	11	NULL	NULL	0	NULL	phosphate	NonProteinOrNucleicAcidChemical	parotid gland	transports via					Na + coupled transporter	Protein				NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism of the transport of phosphate in the intestine is via a proton symporter whilst in the parotid gland it is effected by a Na + coupled transporter .	manualset1
81873	1	387642	11	NULL	NULL	0	NULL	12-O-tetradecanoylphorbol 13-acetate	NonProteinOrNucleicAcidChemical		induces					 inflammation	BiologicalProcess	psoriasis-like			NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism underlying this increased sensitivity of Pglyrp2 ( - / - ) mice to 12-O-tetradecanoylphorbol 13-acetate-induced psoriasis-like inflammation is reduced recruitment of regulatory T cells to the skin and enhanced production and activation of Th17 cells in the skin in Pglyrp2 ( - / - ) mice , which results in more severe inflammation and keratinocyte proliferation .	manualset1
81874	2	387642	11	NULL	NULL	0	NULL	Pglyrp2 ( - / - ) mice	Organism		is sensitivity to					statement 1	process				NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism underlying this increased sensitivity of Pglyrp2 ( - / - ) mice to 12-O-tetradecanoylphorbol 13-acetate-induced psoriasis-like inflammation is reduced recruitment of regulatory T cells to the skin and enhanced production and activation of Th17 cells in the skin in Pglyrp2 ( - / - ) mice , which results in more severe inflammation and keratinocyte proliferation .	manualset1
81875	3	387642	11	NULL	NULL	0	NULL	T cells	cell	regulatory 	recruited to					skin 	Body part				NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism underlying this increased sensitivity of Pglyrp2 ( - / - ) mice to 12-O-tetradecanoylphorbol 13-acetate-induced psoriasis-like inflammation is reduced recruitment of regulatory T cells to the skin and enhanced production and activation of Th17 cells in the skin in Pglyrp2 ( - / - ) mice , which results in more severe inflammation and keratinocyte proliferation .	manualset1
81876	4	387642	11	NULL	NULL	0	NULL	statement 3	BiologicalProcess		produces					Th17 cells	cells	skin			NULL	Pglyrp2 ( - / - ) mice	0	NULL	NULL	NULL	NULL	NULL	The mechanism underlying this increased sensitivity of Pglyrp2 ( - / - ) mice to 12-O-tetradecanoylphorbol 13-acetate-induced psoriasis-like inflammation is reduced recruitment of regulatory T cells to the skin and enhanced production and activation of Th17 cells in the skin in Pglyrp2 ( - / - ) mice , which results in more severe inflammation and keratinocyte proliferation .	manualset1
81877	5	387642	11	NULL	NULL	0	NULL	statement 3	BiologicalProcess		activates					Th17 cell	cells	skin			NULL	Pglyrp2 ( - / - ) mice	0	NULL	NULL	NULL	NULL	NULL	The mechanism underlying this increased sensitivity of Pglyrp2 ( - / - ) mice to 12-O-tetradecanoylphorbol 13-acetate-induced psoriasis-like inflammation is reduced recruitment of regulatory T cells to the skin and enhanced production and activation of Th17 cells in the skin in Pglyrp2 ( - / - ) mice , which results in more severe inflammation and keratinocyte proliferation .	manualset1
81878	6	387642	11	NULL	NULL	0	NULL	statement 4	BiologicalProcess		occurs along with					statement 5	BiologicalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism underlying this increased sensitivity of Pglyrp2 ( - / - ) mice to 12-O-tetradecanoylphorbol 13-acetate-induced psoriasis-like inflammation is reduced recruitment of regulatory T cells to the skin and enhanced production and activation of Th17 cells in the skin in Pglyrp2 ( - / - ) mice , which results in more severe inflammation and keratinocyte proliferation .	manualset1
81879	7	387642	11	NULL	NULL	0	NULL	statement 6	BiologicalProcess		results in					inflammation	BiologicalProcess	severe			NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism underlying this increased sensitivity of Pglyrp2 ( - / - ) mice to 12-O-tetradecanoylphorbol 13-acetate-induced psoriasis-like inflammation is reduced recruitment of regulatory T cells to the skin and enhanced production and activation of Th17 cells in the skin in Pglyrp2 ( - / - ) mice , which results in more severe inflammation and keratinocyte proliferation .	manualset1
81880	8	387642	11	NULL	NULL	0	NULL	statement 6	BiologicalProcess		results in					proliferation	BiologicalProcess	keratinocyte 			NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism underlying this increased sensitivity of Pglyrp2 ( - / - ) mice to 12-O-tetradecanoylphorbol 13-acetate-induced psoriasis-like inflammation is reduced recruitment of regulatory T cells to the skin and enhanced production and activation of Th17 cells in the skin in Pglyrp2 ( - / - ) mice , which results in more severe inflammation and keratinocyte proliferation .	manualset1
81881	1	387644	11	NULL	NULL	0	NULL	electrotransfer	MolecularProcess	DNA	include					electropermeabilization	MolecularProcess	cell			NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanisms involved in DNA electrotransfer , which include cell electropermeabilization and DNA electrophoresis , are also surveyed .	manualset1
81882	2	387644	11	NULL	NULL	0	NULL	electrotransfer	MolecularProcess	DNA	include					electrophoresis	MolecularProcess	DNA			NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanisms involved in DNA electrotransfer , which include cell electropermeabilization and DNA electrophoresis , are also surveyed .	manualset1
81887	1	387668	11	NULL	NULL	0	NULL	melanocortin-1 receptor gene	Gene		undergoes					polymorphism	BiologicalProcess				NULL		0	NULL	NULL	NULL	NULL	NULL	The melanocortin-1 receptor gene polymorphism and association with human skin cancer .	manualset1
81889	2	387668	11	NULL	NULL	0	NULL	statement 1	BiologicalProcess		associated with		may			skin cancer	MedicalFinding	human			NULL		0	NULL	NULL	NULL	NULL	NULL	The melanocortin-1 receptor gene polymorphism and association with human skin cancer .	manualset1
81890	1	387669	11	NULL	NULL	0	NULL	regulators of G-protein signaling	Protein		act as					GTPase-activating protein	Protein	Galpha subunit;;in vitro			NULL		0	NULL	NULL	NULL	NULL	NULL	The members of a recently identified protein family termed regulators of G-protein signaling ( RGS ) act as GTPase-activating proteins for certain Galpha subunits in vitro , but their physiological effects in cells are uncertain in the face of similar biochemical activity and overlapping patterns of tissue expression .	manualset1
81891	1	387670	11	NULL	NULL	0	NULL	humidifier	Chemical	membrane	produces					humidification	MolecularProcess	good			NULL		0	NULL	NULL	NULL	NULL	NULL	The membrane humidifier could produce good humidification .	manualset1
81892	1	387676	11	NULL	NULL	0	NULL	messenger RNA	NucleicAcid	outer membrane protein	are more stable than					messenger RNA	NucleicAcid	bulk of			NULL	 E. coli 	0	NULL	NULL	NULL	NULL	NULL	The messenger RNAs for the outer membrane proteins in E. coli are more stable than the bulk of the messenger RNA s ( Hirashima et al. , 1973 ) .	manualset1
81894	1	387682	11	NULL	NULL	0	NULL	phenobarbital	NonProteinOrNucleicAcidChemical		induce					microsomes	CellComponent	rat liver 			NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolism of Odapipam has been studied with phenobarbital-induced rat liver microsomes , followed by analysis with normal-phase hplc in combination with particle-beam mass spectrometry .	manualset1
81895	1	387683	11	NULL	NULL	0	NULL	rat	Organism		metabolise					pteroylglutamic acid	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolism of pteroylglutamic acid by the rat .	manualset1
81896	1	387688	11	NULL	NULL	0	NULL	metal sites	CellComponent	sarcoplasmic reticulum membrane	bind		highest affinity			lanthanide ions	Ion				NULL		0	NULL	NULL	NULL	NULL	NULL	The metal sites on sarcoplasmic reticulum membranes that bind lanthanide ions with the highest affinity are not the ATPase Ca2 + transport sites .	manualset1
81902	1	387743	11	NULL	NULL	0	NULL	methoxy methyl group	NonProteinOrNucleicAcidChemical	MTBE	 oxidized to					formaldehyde	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The methoxy methyl group of MTBE was oxidized to formaldehyde and ultimately to CO2 .	manualset1
81903	2	387743	11	NULL	NULL	0	NULL	formaldehyde	NonProteinOrNucleicAcidChemical		converted into					CO2	NonProteinOrNucleicAcidChemical				NULL		0	NULL	NULL	NULL	NULL	NULL	The methoxy methyl group of MTBE was oxidized to formaldehyde and ultimately to CO2 .	manualset1
81904	1	387744	11	NULL	NULL	0	NULL	methyl substitution	MolecularProcess	C9;;C10	increased the expression of					T antigen	Protein	adenovirus infected cells			NULL		0	NULL	NULL	NULL	NULL	NULL	The methyl substitution at positions C9 or C10 increased the T antigen expression of adenovirus infected cells .	manualset1
81905	1	387745	11	NULL	NULL	0	NULL	mice	Organism	early postnatal	sensitive to					radiation	EnvironmentalFactor				NULL		0	NULL	NULL	NULL	NULL	NULL	The mice in the early postnatal period were most sensitive to the life-shortening effect of radiation .	manualset1
82033	1	397631	5	NULL	NULL	NULL	NULL	( NHC ) AuCl ) complexes	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( ( NHC ) AuCl ) complexes ( NHC = N-heterocyclic carbene ) , in conjunction with a silver salt , were found to efficiently catalyze the rearrangement of allylic acetates under both conventional and microwave-assisted heating .
	manualset2
82035	3	397631	5	NULL	NULL	NULL	NULL	N-heterocyclic carbene	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( ( NHC ) AuCl ) complexes ( NHC = N-heterocyclic carbene ) , in conjunction with a silver salt , were found to efficiently catalyze the rearrangement of allylic acetates under both conventional and microwave-assisted heating .
	manualset2
82036	4	397631	5	NULL	NULL	NULL	NULL	silver salt	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( ( NHC ) AuCl ) complexes ( NHC = N-heterocyclic carbene ) , in conjunction with a silver salt , were found to efficiently catalyze the rearrangement of allylic acetates under both conventional and microwave-assisted heating .
	manualset2
82037	5	397631	5	NULL	NULL	0	NULL	rearrangement	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( ( NHC ) AuCl ) complexes ( NHC = N-heterocyclic carbene ) , in conjunction with a silver salt , were found to efficiently catalyze the rearrangement of allylic acetates under both conventional and microwave-assisted heating .
	manualset2
82038	6	397631	5	NULL	NULL	NULL	NULL	allylic acetates	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( ( NHC ) AuCl ) complexes ( NHC = N-heterocyclic carbene ) , in conjunction with a silver salt , were found to efficiently catalyze the rearrangement of allylic acetates under both conventional and microwave-assisted heating .
	manualset2
82039	7	397631	5	NULL	NULL	0	NULL	heating	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	( ( NHC ) AuCl ) complexes ( NHC = N-heterocyclic carbene ) , in conjunction with a silver salt , were found to efficiently catalyze the rearrangement of allylic acetates under both conventional and microwave-assisted heating .
	manualset2
82547	2	397631	5	NULL	NULL	0	NULL	NHC	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	( ( NHC ) AuCl ) complexes ( NHC = N-heterocyclic carbene ) , in conjunction with a silver salt , were found to efficiently catalyze the rearrangement of allylic acetates under both conventional and microwave-assisted heating .
	manualset2
82040	1	397632	5	NULL	NULL	0	NULL	Germapect	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( 1st experiences with the antitussive Germapect in the treatment of pulmonary tuberculosis ) .
	manualset2
82041	2	397632	5	NULL	NULL	NULL	NULL	treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( 1st experiences with the antitussive Germapect in the treatment of pulmonary tuberculosis ) .
	manualset2
82042	3	397632	5	NULL	NULL	NULL	NULL	pulmonary tuberculosis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( 1st experiences with the antitussive Germapect in the treatment of pulmonary tuberculosis ) .
	manualset2
82043	1	397633	5	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Advances in the treatment of algodystrophy ) .
	manualset2
82044	2	397633	5	NULL	NULL	0	NULL	algodystrophy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Advances in the treatment of algodystrophy ) .
	manualset2
82045	1	397634	5	NULL	NULL	NULL	NULL	CMV DNA levels	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , CMV DNA levels were consistently higher when targeted at the smaller amplicon , providing additional evidence for the fragmentation of viral DNA .
	manualset2
82047	2	397634	5	NULL	NULL	NULL	NULL	amplicon	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , CMV DNA levels were consistently higher when targeted at the smaller amplicon , providing additional evidence for the fragmentation of viral DNA .
	manualset2
82048	3	397634	5	NULL	NULL	NULL	NULL	fragmentation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , CMV DNA levels were consistently higher when targeted at the smaller amplicon , providing additional evidence for the fragmentation of viral DNA .
	manualset2
82049	4	397634	5	NULL	NULL	NULL	NULL	viral DNA	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , CMV DNA levels were consistently higher when targeted at the smaller amplicon , providing additional evidence for the fragmentation of viral DNA .
	manualset2
82050	1	397635	5	NULL	NULL	0	NULL	CSF	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , CSF increases in the left Sylvian fissure were negatively correlated with the reduction percentage of depressive symptoms at discharge .
	manualset2
82051	2	397635	5	NULL	NULL	NULL	NULL	Sylvian fissure	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , CSF increases in the left Sylvian fissure were negatively correlated with the reduction percentage of depressive symptoms at discharge .
	manualset2
82052	3	397635	5	NULL	NULL	NULL	NULL	depressive symptoms	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , CSF increases in the left Sylvian fissure were negatively correlated with the reduction percentage of depressive symptoms at discharge .
	manualset2
82053	1	397636	5	NULL	NULL	NULL	NULL	Chinese hamster	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , Chinese hamster V79 lung fibroblasts depleted of glutathione display enhanced cytotoxicity on exposure to NO. ( ABSTRACT TRUNCATED AT 250 WORDS )
	manualset2
82054	2	397636	5	NULL	NULL	NULL	NULL	V79 lung fibroblasts	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , Chinese hamster V79 lung fibroblasts depleted of glutathione display enhanced cytotoxicity on exposure to NO. ( ABSTRACT TRUNCATED AT 250 WORDS )
	manualset2
82057	3	397636	5	NULL	NULL	NULL	NULL	glutathione	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , Chinese hamster V79 lung fibroblasts depleted of glutathione display enhanced cytotoxicity on exposure to NO. ( ABSTRACT TRUNCATED AT 250 WORDS )
	manualset2
82058	4	397636	5	NULL	NULL	NULL	NULL	cytotoxicity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , Chinese hamster V79 lung fibroblasts depleted of glutathione display enhanced cytotoxicity on exposure to NO. ( ABSTRACT TRUNCATED AT 250 WORDS )
	manualset2
82548	5	397636	5	NULL	NULL	0	NULL	exposure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , Chinese hamster V79 lung fibroblasts depleted of glutathione display enhanced cytotoxicity on exposure to NO. ( ABSTRACT TRUNCATED AT 250 WORDS )
	manualset2
81909	1	397637	5	NULL	NULL	0	NULL	EDCL	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , EDCL did not alter the expression of bax in HepG2 cells but did selectively downregulate the expression of bcl-2 and bcl-xl , resulting in an increase in the ratio of bax : bcl-2 and bax : bcl-xl .
	manualset2
81910	3	397637	5	NULL	NULL	NULL	NULL	bax	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , EDCL did not alter the expression of bax in HepG2 cells but did selectively downregulate the expression of bcl-2 and bcl-xl , resulting in an increase in the ratio of bax : bcl-2 and bax : bcl-xl .
	manualset2
81911	4	397637	5	NULL	NULL	NULL	NULL	HepG2	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , EDCL did not alter the expression of bax in HepG2 cells but did selectively downregulate the expression of bcl-2 and bcl-xl , resulting in an increase in the ratio of bax : bcl-2 and bax : bcl-xl .
	manualset2
81912	5	397637	5	NULL	NULL	NULL	NULL	bcl-2	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , EDCL did not alter the expression of bax in HepG2 cells but did selectively downregulate the expression of bcl-2 and bcl-xl , resulting in an increase in the ratio of bax : bcl-2 and bax : bcl-xl .
	manualset2
81913	6	397637	5	NULL	NULL	NULL	NULL	bcl-xl	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , EDCL did not alter the expression of bax in HepG2 cells but did selectively downregulate the expression of bcl-2 and bcl-xl , resulting in an increase in the ratio of bax : bcl-2 and bax : bcl-xl .
	manualset2
81954	7	397637	5	NULL	NULL	NULL	NULL	bax : bcl-2	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , EDCL did not alter the expression of bax in HepG2 cells but did selectively downregulate the expression of bcl-2 and bcl-xl , resulting in an increase in the ratio of bax : bcl-2 and bax : bcl-xl .
	manualset2
81955	8	397637	5	NULL	NULL	NULL	NULL	bax : bcl-xl	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , EDCL did not alter the expression of bax in HepG2 cells but did selectively downregulate the expression of bcl-2 and bcl-xl , resulting in an increase in the ratio of bax : bcl-2 and bax : bcl-xl .
	manualset2
82549	2	397637	5	NULL	NULL	0	NULL	expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , EDCL did not alter the expression of bax in HepG2 cells but did selectively downregulate the expression of bcl-2 and bcl-xl , resulting in an increase in the ratio of bax : bcl-2 and bax : bcl-xl .
	manualset2
81914	1	397638	5	NULL	NULL	NULL	NULL	IFN-alpha	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , IFN-alpha markedly induced a 4.7-kb transcript that hybridized to a PKC-epsilon-specific , but not to a PKC-eta-specific , cDNA probe .
	manualset2
81919	3	397638	5	NULL	NULL	NULL	NULL	cDNA probe	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , IFN-alpha markedly induced a 4.7-kb transcript that hybridized to a PKC-epsilon-specific , but not to a PKC-eta-specific , cDNA probe .
	manualset2
82531	2	397638	5	NULL	NULL	NULL	NULL	4.7-kb transcript	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , IFN-alpha markedly induced a 4.7-kb transcript that hybridized to a PKC-epsilon-specific , but not to a PKC-eta-specific , cDNA probe .
	manualset2
81920	1	397639	5	NULL	NULL	NULL	NULL	L-1MT addition	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , L-1MT addition allowed C. trachomatis to undergo secondary differentiation , albeit with limited productive multiplication of the bacterium .
	manualset2
81921	2	397639	5	NULL	NULL	NULL	NULL	C. trachomatis	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , L-1MT addition allowed C. trachomatis to undergo secondary differentiation , albeit with limited productive multiplication of the bacterium .
	manualset2
81922	3	397639	5	NULL	NULL	NULL	NULL	secondary differentiation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , L-1MT addition allowed C. trachomatis to undergo secondary differentiation , albeit with limited productive multiplication of the bacterium .
	manualset2
81923	5	397639	5	NULL	NULL	NULL	NULL	bacterium	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , L-1MT addition allowed C. trachomatis to undergo secondary differentiation , albeit with limited productive multiplication of the bacterium .
	manualset2
81956	4	397639	5	NULL	NULL	NULL	NULL	productive multiplication	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , L-1MT addition allowed C. trachomatis to undergo secondary differentiation , albeit with limited productive multiplication of the bacterium .
	manualset2
81924	1	397640	5	NULL	NULL	NULL	NULL	NKT cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , NKT cells from mice pre-challenged with alpha-GalCer in vivo showed little cytokine production and reduced proliferation in vitro .
	manualset2
81925	2	397640	5	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , NKT cells from mice pre-challenged with alpha-GalCer in vivo showed little cytokine production and reduced proliferation in vitro .
	manualset2
81926	3	397640	5	NULL	NULL	NULL	NULL	alpha-GalCer	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , NKT cells from mice pre-challenged with alpha-GalCer in vivo showed little cytokine production and reduced proliferation in vitro .
	manualset2
81927	4	397640	5	NULL	NULL	NULL	NULL	cytokine production	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , NKT cells from mice pre-challenged with alpha-GalCer in vivo showed little cytokine production and reduced proliferation in vitro .
	manualset2
81928	5	397640	5	NULL	NULL	NULL	NULL	reduced proliferation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , NKT cells from mice pre-challenged with alpha-GalCer in vivo showed little cytokine production and reduced proliferation in vitro .
	manualset2
81929	1	397641	5	NULL	NULL	0	NULL	RASSF6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , RASSF6 is often downregulated in primary human tumors .
	manualset2
81930	2	397641	5	NULL	NULL	NULL	NULL	human tumors	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , RASSF6 is often downregulated in primary human tumors .
	manualset2
81932	1	397642	5	NULL	NULL	NULL	NULL	TLR activation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , TLR activation is capable of modulating the adaptive immune response with a bias towards a Th1 T-cell response .
	manualset2
81935	2	397642	5	NULL	NULL	NULL	NULL	adaptive immune response	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , TLR activation is capable of modulating the adaptive immune response with a bias towards a Th1 T-cell response .
	manualset2
81936	3	397642	5	NULL	NULL	NULL	NULL	Th1 T-cell response	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , TLR activation is capable of modulating the adaptive immune response with a bias towards a Th1 T-cell response .
	manualset2
81937	2	397643	5	NULL	NULL	NULL	NULL	diabetes-induced alterations	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , Western blot data indicated that the diabetes-induced alterations in the cardiac ryanodine receptor Ca ( 2 + ) release channel 's hyperphosphorylation decreased the FKBP12 .6 protein level .
	manualset2
81938	4	397643	5	NULL	NULL	NULL	NULL	Ca ( 2 + ) release channel	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , Western blot data indicated that the diabetes-induced alterations in the cardiac ryanodine receptor Ca ( 2 + ) release channel 's hyperphosphorylation decreased the FKBP12 .6 protein level .
	manualset2
81941	5	397643	5	NULL	NULL	NULL	NULL	hyperphosphorylation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , Western blot data indicated that the diabetes-induced alterations in the cardiac ryanodine receptor Ca ( 2 + ) release channel 's hyperphosphorylation decreased the FKBP12 .6 protein level .
	manualset2
81942	6	397643	5	NULL	NULL	NULL	NULL	FKBP12 .6 protein level	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , Western blot data indicated that the diabetes-induced alterations in the cardiac ryanodine receptor Ca ( 2 + ) release channel 's hyperphosphorylation decreased the FKBP12 .6 protein level .
	manualset2
81960	1	397643	5	NULL	NULL	NULL	NULL	Western blot data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , Western blot data indicated that the diabetes-induced alterations in the cardiac ryanodine receptor Ca ( 2 + ) release channel 's hyperphosphorylation decreased the FKBP12 .6 protein level .
	manualset2
81961	3	397643	5	NULL	NULL	NULL	NULL	cardiac ryanodine receptor	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , Western blot data indicated that the diabetes-induced alterations in the cardiac ryanodine receptor Ca ( 2 + ) release channel 's hyperphosphorylation decreased the FKBP12 .6 protein level .
	manualset2
81943	2	397644	5	NULL	NULL	NULL	NULL	adult stem cell population	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , ablation of the adult stem cell population leads to concomitant loss of PBK/TOPK-positive cells in the SEZ .
	manualset2
81944	4	397644	5	NULL	NULL	NULL	NULL	PBK/TOPK-positive cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , ablation of the adult stem cell population leads to concomitant loss of PBK/TOPK-positive cells in the SEZ .
	manualset2
81945	5	397644	5	NULL	NULL	NULL	NULL	SEZ	AnatomicalPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , ablation of the adult stem cell population leads to concomitant loss of PBK/TOPK-positive cells in the SEZ .
	manualset2
81946	1	397644	5	NULL	NULL	NULL	NULL	ablation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , ablation of the adult stem cell population leads to concomitant loss of PBK/TOPK-positive cells in the SEZ .
	manualset2
81963	3	397644	5	NULL	NULL	NULL	NULL	concomitant loss	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , ablation of the adult stem cell population leads to concomitant loss of PBK/TOPK-positive cells in the SEZ .
	manualset2
81947	1	397645	5	NULL	NULL	NULL	NULL	pseudo-PBs	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , abnormally large pseudo-PBs , as large as four times the normal PB sizes , were observed .
	manualset2
81965	2	397645	5	NULL	NULL	0	NULL	PB	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , abnormally large pseudo-PBs , as large as four times the normal PB sizes , were observed .
	manualset2
81948	3	397646	5	NULL	NULL	NULL	NULL	intracellular free Ca ( 2 + )	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , activation of these receptors was found to increase the steady-state level of intracellular free Ca ( 2 + ) in EECs and the frequency of beating of cardiomyocytes .
	manualset2
81949	4	397646	5	NULL	NULL	NULL	NULL	EECs	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , activation of these receptors was found to increase the steady-state level of intracellular free Ca ( 2 + ) in EECs and the frequency of beating of cardiomyocytes .
	manualset2
81967	1	397646	5	NULL	NULL	0	NULL	activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , activation of these receptors was found to increase the steady-state level of intracellular free Ca ( 2 + ) in EECs and the frequency of beating of cardiomyocytes .
	manualset2
81968	2	397646	5	NULL	NULL	0	NULL	receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , activation of these receptors was found to increase the steady-state level of intracellular free Ca ( 2 + ) in EECs and the frequency of beating of cardiomyocytes .
	manualset2
81971	5	397646	5	NULL	NULL	NULL	NULL	beating	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , activation of these receptors was found to increase the steady-state level of intracellular free Ca ( 2 + ) in EECs and the frequency of beating of cardiomyocytes .
	manualset2
82555	6	397646	5	NULL	NULL	0	NULL	cardiomyocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , activation of these receptors was found to increase the steady-state level of intracellular free Ca ( 2 + ) in EECs and the frequency of beating of cardiomyocytes .
	manualset2
81972	1	397647	5	NULL	NULL	NULL	NULL	adoptive transfer experiments	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , adoptive transfer experiments have revealed that activated liver lymphocytes may migrate to other organs to inhibit tumor growth , such as the lungs and kidneys .
	manualset2
81973	2	397647	5	NULL	NULL	NULL	NULL	activated liver lymphocytes	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , adoptive transfer experiments have revealed that activated liver lymphocytes may migrate to other organs to inhibit tumor growth , such as the lungs and kidneys .
	manualset2
81976	3	397647	5	NULL	NULL	NULL	NULL	organs	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , adoptive transfer experiments have revealed that activated liver lymphocytes may migrate to other organs to inhibit tumor growth , such as the lungs and kidneys .
	manualset2
81977	4	397647	5	NULL	NULL	NULL	NULL	tumor growth	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , adoptive transfer experiments have revealed that activated liver lymphocytes may migrate to other organs to inhibit tumor growth , such as the lungs and kidneys .
	manualset2
81979	5	397647	5	NULL	NULL	NULL	NULL	lungs	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , adoptive transfer experiments have revealed that activated liver lymphocytes may migrate to other organs to inhibit tumor growth , such as the lungs and kidneys .
	manualset2
81980	6	397647	5	NULL	NULL	NULL	NULL	kidneys	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , adoptive transfer experiments have revealed that activated liver lymphocytes may migrate to other organs to inhibit tumor growth , such as the lungs and kidneys .
	manualset2
81981	1	397648	5	NULL	NULL	0	NULL	airway remodeling	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , airway remodeling changes were significantly reduced with TSA compared to vehicle-treated mice , with fewer goblet cells ( p & lt ; 0.05 ) , less subepithelial collagen deposition ( p & lt ; 0.05 ) and attenuated airway hyperresponsiveness at the highest methacholine dose .
	manualset2
81982	2	397648	5	NULL	NULL	0	NULL	TSA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , airway remodeling changes were significantly reduced with TSA compared to vehicle-treated mice , with fewer goblet cells ( p & lt ; 0.05 ) , less subepithelial collagen deposition ( p & lt ; 0.05 ) and attenuated airway hyperresponsiveness at the highest methacholine dose .
	manualset2
81983	3	397648	5	NULL	NULL	NULL	NULL	 vehicle-treated mice	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , airway remodeling changes were significantly reduced with TSA compared to vehicle-treated mice , with fewer goblet cells ( p & lt ; 0.05 ) , less subepithelial collagen deposition ( p & lt ; 0.05 ) and attenuated airway hyperresponsiveness at the highest methacholine dose .
	manualset2
81984	4	397648	5	NULL	NULL	0	NULL	goblet cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , airway remodeling changes were significantly reduced with TSA compared to vehicle-treated mice , with fewer goblet cells ( p & lt ; 0.05 ) , less subepithelial collagen deposition ( p & lt ; 0.05 ) and attenuated airway hyperresponsiveness at the highest methacholine dose .
	manualset2
81985	5	397648	5	NULL	NULL	NULL	NULL	subepithelial collagen deposition	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , airway remodeling changes were significantly reduced with TSA compared to vehicle-treated mice , with fewer goblet cells ( p & lt ; 0.05 ) , less subepithelial collagen deposition ( p & lt ; 0.05 ) and attenuated airway hyperresponsiveness at the highest methacholine dose .
	manualset2
81987	6	397648	5	NULL	NULL	NULL	NULL	airway hyperresponsiveness	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , airway remodeling changes were significantly reduced with TSA compared to vehicle-treated mice , with fewer goblet cells ( p & lt ; 0.05 ) , less subepithelial collagen deposition ( p & lt ; 0.05 ) and attenuated airway hyperresponsiveness at the highest methacholine dose .
	manualset2
81988	7	397648	5	NULL	NULL	NULL	NULL	methacholine	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , airway remodeling changes were significantly reduced with TSA compared to vehicle-treated mice , with fewer goblet cells ( p & lt ; 0.05 ) , less subepithelial collagen deposition ( p & lt ; 0.05 ) and attenuated airway hyperresponsiveness at the highest methacholine dose .
	manualset2
81989	1	397649	5	NULL	NULL	0	NULL	acetic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , an interesting effect of acetic acid as an additive is uncovered that facilitates catalyst activation .
	manualset2
81990	2	397649	5	NULL	NULL	NULL	NULL	catalyst activation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , an interesting effect of acetic acid as an additive is uncovered that facilitates catalyst activation .
	manualset2
81992	1	397650	5	NULL	NULL	NULL	NULL	tissue factor	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Role of tissue factor in atherothrombosis ) .
	manualset2
81993	2	397650	5	NULL	NULL	0	NULL	atherothrombosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Role of tissue factor in atherothrombosis ) .
	manualset2
81994	1	397651	5	NULL	NULL	NULL	NULL	phytohemagglutinin ( PHA ) - activated T-cell lysates	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , analysis of phytohemagglutinin ( PHA ) - activated T-cell lysates for LHRH by RIA demonstrated that the mean concentration of LHRH in PHA-activated T-cells increased from 45 + / - 4.5 to 64 + / - 7 pg/10 ( 6 ) cells after 24 h of culture and from 47 + / - 3.6 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.01 ) after 48 h. While the LHRH concentration in PHA-activated cells increased over the last 24 h of culture h from 64 + / - 7 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.001 ) , there was no change in mean concentration of LHRH in T-cells kept in medium alone .
	manualset2
81998	2	397651	5	NULL	NULL	NULL	NULL	LHRH	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , analysis of phytohemagglutinin ( PHA ) - activated T-cell lysates for LHRH by RIA demonstrated that the mean concentration of LHRH in PHA-activated T-cells increased from 45 + / - 4.5 to 64 + / - 7 pg/10 ( 6 ) cells after 24 h of culture and from 47 + / - 3.6 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.01 ) after 48 h. While the LHRH concentration in PHA-activated cells increased over the last 24 h of culture h from 64 + / - 7 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.001 ) , there was no change in mean concentration of LHRH in T-cells kept in medium alone .
	manualset2
81999	3	397651	5	NULL	NULL	NULL	NULL	RIA	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , analysis of phytohemagglutinin ( PHA ) - activated T-cell lysates for LHRH by RIA demonstrated that the mean concentration of LHRH in PHA-activated T-cells increased from 45 + / - 4.5 to 64 + / - 7 pg/10 ( 6 ) cells after 24 h of culture and from 47 + / - 3.6 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.01 ) after 48 h. While the LHRH concentration in PHA-activated cells increased over the last 24 h of culture h from 64 + / - 7 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.001 ) , there was no change in mean concentration of LHRH in T-cells kept in medium alone .
	manualset2
82000	4	397651	5	NULL	NULL	NULL	NULL	LHRH	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , analysis of phytohemagglutinin ( PHA ) - activated T-cell lysates for LHRH by RIA demonstrated that the mean concentration of LHRH in PHA-activated T-cells increased from 45 + / - 4.5 to 64 + / - 7 pg/10 ( 6 ) cells after 24 h of culture and from 47 + / - 3.6 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.01 ) after 48 h. While the LHRH concentration in PHA-activated cells increased over the last 24 h of culture h from 64 + / - 7 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.001 ) , there was no change in mean concentration of LHRH in T-cells kept in medium alone .
	manualset2
82059	6	397651	5	NULL	NULL	NULL	NULL	45 + / - 4.5 pg/10 ( 6 ) cells	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , analysis of phytohemagglutinin ( PHA ) - activated T-cell lysates for LHRH by RIA demonstrated that the mean concentration of LHRH in PHA-activated T-cells increased from 45 + / - 4.5 to 64 + / - 7 pg/10 ( 6 ) cells after 24 h of culture and from 47 + / - 3.6 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.01 ) after 48 h. While the LHRH concentration in PHA-activated cells increased over the last 24 h of culture h from 64 + / - 7 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.001 ) , there was no change in mean concentration of LHRH in T-cells kept in medium alone .
	manualset2
82060	7	397651	5	NULL	NULL	NULL	NULL	64 + / - 7 pg/10 ( 6 ) cells	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , analysis of phytohemagglutinin ( PHA ) - activated T-cell lysates for LHRH by RIA demonstrated that the mean concentration of LHRH in PHA-activated T-cells increased from 45 + / - 4.5 to 64 + / - 7 pg/10 ( 6 ) cells after 24 h of culture and from 47 + / - 3.6 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.01 ) after 48 h. While the LHRH concentration in PHA-activated cells increased over the last 24 h of culture h from 64 + / - 7 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.001 ) , there was no change in mean concentration of LHRH in T-cells kept in medium alone .
	manualset2
82062	8	397651	5	NULL	NULL	NULL	NULL	24 h	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , analysis of phytohemagglutinin ( PHA ) - activated T-cell lysates for LHRH by RIA demonstrated that the mean concentration of LHRH in PHA-activated T-cells increased from 45 + / - 4.5 to 64 + / - 7 pg/10 ( 6 ) cells after 24 h of culture and from 47 + / - 3.6 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.01 ) after 48 h. While the LHRH concentration in PHA-activated cells increased over the last 24 h of culture h from 64 + / - 7 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.001 ) , there was no change in mean concentration of LHRH in T-cells kept in medium alone .
	manualset2
82063	9	397651	5	NULL	NULL	NULL	NULL	47 + / - 3.6 pg/10 ( 6 ) cells	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , analysis of phytohemagglutinin ( PHA ) - activated T-cell lysates for LHRH by RIA demonstrated that the mean concentration of LHRH in PHA-activated T-cells increased from 45 + / - 4.5 to 64 + / - 7 pg/10 ( 6 ) cells after 24 h of culture and from 47 + / - 3.6 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.01 ) after 48 h. While the LHRH concentration in PHA-activated cells increased over the last 24 h of culture h from 64 + / - 7 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.001 ) , there was no change in mean concentration of LHRH in T-cells kept in medium alone .
	manualset2
82064	10	397651	5	NULL	NULL	NULL	NULL	117 + / - 11.8 pg/10 ( 6 ) cells	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , analysis of phytohemagglutinin ( PHA ) - activated T-cell lysates for LHRH by RIA demonstrated that the mean concentration of LHRH in PHA-activated T-cells increased from 45 + / - 4.5 to 64 + / - 7 pg/10 ( 6 ) cells after 24 h of culture and from 47 + / - 3.6 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.01 ) after 48 h. While the LHRH concentration in PHA-activated cells increased over the last 24 h of culture h from 64 + / - 7 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.001 ) , there was no change in mean concentration of LHRH in T-cells kept in medium alone .
	manualset2
82066	11	397651	5	NULL	NULL	NULL	NULL	48 h	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , analysis of phytohemagglutinin ( PHA ) - activated T-cell lysates for LHRH by RIA demonstrated that the mean concentration of LHRH in PHA-activated T-cells increased from 45 + / - 4.5 to 64 + / - 7 pg/10 ( 6 ) cells after 24 h of culture and from 47 + / - 3.6 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.01 ) after 48 h. While the LHRH concentration in PHA-activated cells increased over the last 24 h of culture h from 64 + / - 7 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.001 ) , there was no change in mean concentration of LHRH in T-cells kept in medium alone .
	manualset2
82067	12	397651	5	NULL	NULL	NULL	NULL	LHRH concentration	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , analysis of phytohemagglutinin ( PHA ) - activated T-cell lysates for LHRH by RIA demonstrated that the mean concentration of LHRH in PHA-activated T-cells increased from 45 + / - 4.5 to 64 + / - 7 pg/10 ( 6 ) cells after 24 h of culture and from 47 + / - 3.6 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.01 ) after 48 h. While the LHRH concentration in PHA-activated cells increased over the last 24 h of culture h from 64 + / - 7 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.001 ) , there was no change in mean concentration of LHRH in T-cells kept in medium alone .
	manualset2
82068	13	397651	5	NULL	NULL	NULL	NULL	PHA-activated cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , analysis of phytohemagglutinin ( PHA ) - activated T-cell lysates for LHRH by RIA demonstrated that the mean concentration of LHRH in PHA-activated T-cells increased from 45 + / - 4.5 to 64 + / - 7 pg/10 ( 6 ) cells after 24 h of culture and from 47 + / - 3.6 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.01 ) after 48 h. While the LHRH concentration in PHA-activated cells increased over the last 24 h of culture h from 64 + / - 7 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.001 ) , there was no change in mean concentration of LHRH in T-cells kept in medium alone .
	manualset2
82070	14	397651	5	NULL	NULL	NULL	NULL	24 h	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , analysis of phytohemagglutinin ( PHA ) - activated T-cell lysates for LHRH by RIA demonstrated that the mean concentration of LHRH in PHA-activated T-cells increased from 45 + / - 4.5 to 64 + / - 7 pg/10 ( 6 ) cells after 24 h of culture and from 47 + / - 3.6 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.01 ) after 48 h. While the LHRH concentration in PHA-activated cells increased over the last 24 h of culture h from 64 + / - 7 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.001 ) , there was no change in mean concentration of LHRH in T-cells kept in medium alone .
	manualset2
82071	15	397651	5	NULL	NULL	NULL	NULL	64 + / - 7 pg/10 ( 6 ) cells	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , analysis of phytohemagglutinin ( PHA ) - activated T-cell lysates for LHRH by RIA demonstrated that the mean concentration of LHRH in PHA-activated T-cells increased from 45 + / - 4.5 to 64 + / - 7 pg/10 ( 6 ) cells after 24 h of culture and from 47 + / - 3.6 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.01 ) after 48 h. While the LHRH concentration in PHA-activated cells increased over the last 24 h of culture h from 64 + / - 7 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.001 ) , there was no change in mean concentration of LHRH in T-cells kept in medium alone .
	manualset2
82072	16	397651	5	NULL	NULL	NULL	NULL	117 + / - 11.8 pg/10 ( 6 ) cells	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , analysis of phytohemagglutinin ( PHA ) - activated T-cell lysates for LHRH by RIA demonstrated that the mean concentration of LHRH in PHA-activated T-cells increased from 45 + / - 4.5 to 64 + / - 7 pg/10 ( 6 ) cells after 24 h of culture and from 47 + / - 3.6 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.01 ) after 48 h. While the LHRH concentration in PHA-activated cells increased over the last 24 h of culture h from 64 + / - 7 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.001 ) , there was no change in mean concentration of LHRH in T-cells kept in medium alone .
	manualset2
82074	17	397651	5	NULL	NULL	NULL	NULL	LHRH 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , analysis of phytohemagglutinin ( PHA ) - activated T-cell lysates for LHRH by RIA demonstrated that the mean concentration of LHRH in PHA-activated T-cells increased from 45 + / - 4.5 to 64 + / - 7 pg/10 ( 6 ) cells after 24 h of culture and from 47 + / - 3.6 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.01 ) after 48 h. While the LHRH concentration in PHA-activated cells increased over the last 24 h of culture h from 64 + / - 7 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.001 ) , there was no change in mean concentration of LHRH in T-cells kept in medium alone .
	manualset2
82075	19	397651	5	NULL	NULL	NULL	NULL	T-cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , analysis of phytohemagglutinin ( PHA ) - activated T-cell lysates for LHRH by RIA demonstrated that the mean concentration of LHRH in PHA-activated T-cells increased from 45 + / - 4.5 to 64 + / - 7 pg/10 ( 6 ) cells after 24 h of culture and from 47 + / - 3.6 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.01 ) after 48 h. While the LHRH concentration in PHA-activated cells increased over the last 24 h of culture h from 64 + / - 7 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.001 ) , there was no change in mean concentration of LHRH in T-cells kept in medium alone .
	manualset2
82556	5	397651	5	NULL	NULL	0	NULL	PHA-activated T-cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , analysis of phytohemagglutinin ( PHA ) - activated T-cell lysates for LHRH by RIA demonstrated that the mean concentration of LHRH in PHA-activated T-cells increased from 45 + / - 4.5 to 64 + / - 7 pg/10 ( 6 ) cells after 24 h of culture and from 47 + / - 3.6 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.01 ) after 48 h. While the LHRH concentration in PHA-activated cells increased over the last 24 h of culture h from 64 + / - 7 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.001 ) , there was no change in mean concentration of LHRH in T-cells kept in medium alone .
	manualset2
82557	18	397651	5	NULL	NULL	0	NULL	T-cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , analysis of phytohemagglutinin ( PHA ) - activated T-cell lysates for LHRH by RIA demonstrated that the mean concentration of LHRH in PHA-activated T-cells increased from 45 + / - 4.5 to 64 + / - 7 pg/10 ( 6 ) cells after 24 h of culture and from 47 + / - 3.6 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.01 ) after 48 h. While the LHRH concentration in PHA-activated cells increased over the last 24 h of culture h from 64 + / - 7 to 117 + / - 11.8 pg/10 ( 6 ) cells ( P & lt ; 0.001 ) , there was no change in mean concentration of LHRH in T-cells kept in medium alone .
	manualset2
82003	2	397652	5	NULL	NULL	NULL	NULL	syndrome	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , as executive functions are thought to be spared in this syndrome , TGA provides an opportunity to examine the impact of a massive `` pure '' memory impairment on PM .
	manualset2
82004	3	397652	5	NULL	NULL	NULL	NULL	TGA	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , as executive functions are thought to be spared in this syndrome , TGA provides an opportunity to examine the impact of a massive `` pure '' memory impairment on PM .
	manualset2
82005	4	397652	5	NULL	NULL	NULL	NULL	memory impairment	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , as executive functions are thought to be spared in this syndrome , TGA provides an opportunity to examine the impact of a massive `` pure '' memory impairment on PM .
	manualset2
82006	5	397652	5	NULL	NULL	NULL	NULL	PM	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , as executive functions are thought to be spared in this syndrome , TGA provides an opportunity to examine the impact of a massive `` pure '' memory impairment on PM .
	manualset2
82550	1	397652	5	NULL	NULL	0	NULL	executive functions	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , as executive functions are thought to be spared in this syndrome , TGA provides an opportunity to examine the impact of a massive `` pure '' memory impairment on PM .
	manualset2
82008	1	397653	5	NULL	NULL	NULL	NULL	bioinformatics analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , bioinformatics analysis predicted an increased significance of binding site clusters in the CRMs of h 1 , eve 1 , run 1 and ftz 1when Hkb was incorporated in the analysis , indicating that Hkb plays a direct role in these CRMs .
	manualset2
82022	2	397653	5	NULL	NULL	NULL	NULL	binding site clusters	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , bioinformatics analysis predicted an increased significance of binding site clusters in the CRMs of h 1 , eve 1 , run 1 and ftz 1when Hkb was incorporated in the analysis , indicating that Hkb plays a direct role in these CRMs .
	manualset2
82024	3	397653	5	NULL	NULL	NULL	NULL	CRMs	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , bioinformatics analysis predicted an increased significance of binding site clusters in the CRMs of h 1 , eve 1 , run 1 and ftz 1when Hkb was incorporated in the analysis , indicating that Hkb plays a direct role in these CRMs .
	manualset2
82025	4	397653	5	NULL	NULL	NULL	NULL	h 1	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , bioinformatics analysis predicted an increased significance of binding site clusters in the CRMs of h 1 , eve 1 , run 1 and ftz 1when Hkb was incorporated in the analysis , indicating that Hkb plays a direct role in these CRMs .
	manualset2
82026	5	397653	5	NULL	NULL	NULL	NULL	eve 1	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , bioinformatics analysis predicted an increased significance of binding site clusters in the CRMs of h 1 , eve 1 , run 1 and ftz 1when Hkb was incorporated in the analysis , indicating that Hkb plays a direct role in these CRMs .
	manualset2
82027	6	397653	5	NULL	NULL	NULL	NULL	run 1	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , bioinformatics analysis predicted an increased significance of binding site clusters in the CRMs of h 1 , eve 1 , run 1 and ftz 1when Hkb was incorporated in the analysis , indicating that Hkb plays a direct role in these CRMs .
	manualset2
82028	7	397653	5	NULL	NULL	NULL	NULL	ftz 1	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , bioinformatics analysis predicted an increased significance of binding site clusters in the CRMs of h 1 , eve 1 , run 1 and ftz 1when Hkb was incorporated in the analysis , indicating that Hkb plays a direct role in these CRMs .
	manualset2
82029	8	397653	5	NULL	NULL	NULL	NULL	Hkb	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , bioinformatics analysis predicted an increased significance of binding site clusters in the CRMs of h 1 , eve 1 , run 1 and ftz 1when Hkb was incorporated in the analysis , indicating that Hkb plays a direct role in these CRMs .
	manualset2
82030	9	397653	5	NULL	NULL	NULL	NULL	analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , bioinformatics analysis predicted an increased significance of binding site clusters in the CRMs of h 1 , eve 1 , run 1 and ftz 1when Hkb was incorporated in the analysis , indicating that Hkb plays a direct role in these CRMs .
	manualset2
82031	10	397653	5	NULL	NULL	NULL	NULL	Hkb	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , bioinformatics analysis predicted an increased significance of binding site clusters in the CRMs of h 1 , eve 1 , run 1 and ftz 1when Hkb was incorporated in the analysis , indicating that Hkb plays a direct role in these CRMs .
	manualset2
82032	11	397653	5	NULL	NULL	NULL	NULL	CRMs	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , bioinformatics analysis predicted an increased significance of binding site clusters in the CRMs of h 1 , eve 1 , run 1 and ftz 1when Hkb was incorporated in the analysis , indicating that Hkb plays a direct role in these CRMs .
	manualset2
82009	1	397654	5	NULL	NULL	NULL	NULL	c-kit mRNA	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , c-kit mRNA and protein were down-regulated during erythroid differentiation .
	manualset2
82010	2	397654	5	NULL	NULL	NULL	NULL	c-kit protein	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , c-kit mRNA and protein were down-regulated during erythroid differentiation .
	manualset2
82012	3	397654	5	NULL	NULL	NULL	NULL	erythroid differentiation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , c-kit mRNA and protein were down-regulated during erythroid differentiation .
	manualset2
82014	1	397655	5	NULL	NULL	NULL	NULL	carbonyl modification	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , carbonyl modification of HCNP-pp may be involved in pathophysiological alterations associated with deterioration in the learning and memory in the brain seen in SAMP8 .
	manualset2
82015	2	397655	5	NULL	NULL	0	NULL	HCNP-pp	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , carbonyl modification of HCNP-pp may be involved in pathophysiological alterations associated with deterioration in the learning and memory in the brain seen in SAMP8 .
	manualset2
82016	3	397655	5	NULL	NULL	NULL	NULL	pathophysiological alterations	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , carbonyl modification of HCNP-pp may be involved in pathophysiological alterations associated with deterioration in the learning and memory in the brain seen in SAMP8 .
	manualset2
82017	4	397655	5	NULL	NULL	0	NULL	deterioration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , carbonyl modification of HCNP-pp may be involved in pathophysiological alterations associated with deterioration in the learning and memory in the brain seen in SAMP8 .
	manualset2
82018	5	397655	5	NULL	NULL	NULL	NULL	learning and memory	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , carbonyl modification of HCNP-pp may be involved in pathophysiological alterations associated with deterioration in the learning and memory in the brain seen in SAMP8 .
	manualset2
82020	6	397655	5	NULL	NULL	NULL	NULL	brain	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , carbonyl modification of HCNP-pp may be involved in pathophysiological alterations associated with deterioration in the learning and memory in the brain seen in SAMP8 .
	manualset2
82021	4	397655	5	NULL	NULL	NULL	NULL	SAMP8	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , carbonyl modification of HCNP-pp may be involved in pathophysiological alterations associated with deterioration in the learning and memory in the brain seen in SAMP8 .
	manualset2
82076	1	397656	5	NULL	NULL	NULL	NULL	cell surface biotinylation experiments	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , cell surface biotinylation experiments showed that - calpain was clearly detected among the cell surface proteins .
	manualset2
82079	2	397656	5	NULL	NULL	NULL	NULL	calpain	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , cell surface biotinylation experiments showed that - calpain was clearly detected among the cell surface proteins .
	manualset2
82080	3	397656	5	NULL	NULL	NULL	NULL	cell surface proteins	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , cell surface biotinylation experiments showed that - calpain was clearly detected among the cell surface proteins .
	manualset2
82083	1	397657	5	NULL	NULL	0	NULL	chemoimmunotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , chemoimmunotherapy containing rituximab has led to significant increases in complete response and progression-free survival rates for patients with both previously untreated and relapsed or refractory chronic lymphocytic leukemia ( CLL ) .
	manualset2
82084	2	397657	5	NULL	NULL	NULL	NULL	rituximab	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , chemoimmunotherapy containing rituximab has led to significant increases in complete response and progression-free survival rates for patients with both previously untreated and relapsed or refractory chronic lymphocytic leukemia ( CLL ) .
	manualset2
82085	3	397657	5	NULL	NULL	0	NULL	response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , chemoimmunotherapy containing rituximab has led to significant increases in complete response and progression-free survival rates for patients with both previously untreated and relapsed or refractory chronic lymphocytic leukemia ( CLL ) .
	manualset2
82086	4	397657	5	NULL	NULL	0	NULL	progression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , chemoimmunotherapy containing rituximab has led to significant increases in complete response and progression-free survival rates for patients with both previously untreated and relapsed or refractory chronic lymphocytic leukemia ( CLL ) .
	manualset2
82087	5	397657	5	NULL	NULL	NULL	NULL	survival rates	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , chemoimmunotherapy containing rituximab has led to significant increases in complete response and progression-free survival rates for patients with both previously untreated and relapsed or refractory chronic lymphocytic leukemia ( CLL ) .
	manualset2
82088	6	397657	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , chemoimmunotherapy containing rituximab has led to significant increases in complete response and progression-free survival rates for patients with both previously untreated and relapsed or refractory chronic lymphocytic leukemia ( CLL ) .
	manualset2
82089	7	397657	5	NULL	NULL	NULL	NULL	refractory chronic lymphocytic leukemia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , chemoimmunotherapy containing rituximab has led to significant increases in complete response and progression-free survival rates for patients with both previously untreated and relapsed or refractory chronic lymphocytic leukemia ( CLL ) .
	manualset2
82090	1	397658	5	NULL	NULL	NULL	NULL	class I-directed cytotoxicity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , class I-directed cytotoxicity failed to develop in the absence of CD4 ( + ) T cells .
	manualset2
82091	2	397658	5	NULL	NULL	NULL	NULL	CD4 ( + ) T cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , class I-directed cytotoxicity failed to develop in the absence of CD4 ( + ) T cells .
	manualset2
82093	1	397659	5	NULL	NULL	0	NULL	co-expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , co-expression of Pax-6 did not enhance promoter activity .
	manualset2
82094	2	397659	5	NULL	NULL	0	NULL	Pax-6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , co-expression of Pax-6 did not enhance promoter activity .
	manualset2
82095	3	397659	5	NULL	NULL	NULL	NULL	promoter activity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , co-expression of Pax-6 did not enhance promoter activity .
	manualset2
82097	1	397660	5	NULL	NULL	0	NULL	competition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , competition between SMILE and the coactivator peroxisome proliferator-activated receptor ( PGC-1 ) on CREBH transactivation has been demonstrated in vitro and in vivo .
	manualset2
82098	2	397660	5	NULL	NULL	0	NULL	SMILE	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , competition between SMILE and the coactivator peroxisome proliferator-activated receptor ( PGC-1 ) on CREBH transactivation has been demonstrated in vitro and in vivo .
	manualset2
82099	3	397660	5	NULL	NULL	NULL	NULL	coactivator peroxisome proliferator-activated receptor ( PGC-1 )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , competition between SMILE and the coactivator peroxisome proliferator-activated receptor ( PGC-1 ) on CREBH transactivation has been demonstrated in vitro and in vivo .
	manualset2
82104	8	397660	5	NULL	NULL	NULL	NULL	CREBH transactivation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , competition between SMILE and the coactivator peroxisome proliferator-activated receptor ( PGC-1 ) on CREBH transactivation has been demonstrated in vitro and in vivo .
	manualset2
82106	1	397661	5	NULL	NULL	NULL	NULL	vitamin E	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Role of vitamin E in adaptation and stress processes in premature infants ) .
	manualset2
82107	2	397661	5	NULL	NULL	NULL	NULL	adaptation and stress processes	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Role of vitamin E in adaptation and stress processes in premature infants ) .
	manualset2
82110	3	397661	5	NULL	NULL	NULL	NULL	premature infants	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Role of vitamin E in adaptation and stress processes in premature infants ) .
	manualset2
82111	1	397662	5	NULL	NULL	NULL	NULL	dDAVP	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , dDAVP potentiated CRF and neither its own ACTH-releasing action nor its potentiation of CRF were sensitive to previous VI - or V2-receptor blockade .
	manualset2
82112	2	397662	5	NULL	NULL	0	NULL	CRF	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , dDAVP potentiated CRF and neither its own ACTH-releasing action nor its potentiation of CRF were sensitive to previous VI - or V2-receptor blockade .
	manualset2
82113	3	397662	5	NULL	NULL	NULL	NULL	ACTH-releasing action	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , dDAVP potentiated CRF and neither its own ACTH-releasing action nor its potentiation of CRF were sensitive to previous VI - or V2-receptor blockade .
	manualset2
82115	4	397662	5	NULL	NULL	NULL	NULL	potentiation of CRF	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , dDAVP potentiated CRF and neither its own ACTH-releasing action nor its potentiation of CRF were sensitive to previous VI - or V2-receptor blockade .
	manualset2
82117	5	397662	5	NULL	NULL	NULL	NULL	VI - or V2-receptor blockade	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , dDAVP potentiated CRF and neither its own ACTH-releasing action nor its potentiation of CRF were sensitive to previous VI - or V2-receptor blockade .
	manualset2
82119	1	397663	5	NULL	NULL	0	NULL	Annexin V	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , double staining with Annexin V and PI revealed that hMTERF4 knockdown increased necrosis but not apoptosis .
	manualset2
82120	2	397663	5	NULL	NULL	0	NULL	PI	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , double staining with Annexin V and PI revealed that hMTERF4 knockdown increased necrosis but not apoptosis .
	manualset2
82121	3	397663	5	NULL	NULL	NULL	NULL	hMTERF4 knockdown	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , double staining with Annexin V and PI revealed that hMTERF4 knockdown increased necrosis but not apoptosis .
	manualset2
82122	4	397663	5	NULL	NULL	NULL	NULL	necrosis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , double staining with Annexin V and PI revealed that hMTERF4 knockdown increased necrosis but not apoptosis .
	manualset2
82123	5	397663	5	NULL	NULL	NULL	NULL	apoptosis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , double staining with Annexin V and PI revealed that hMTERF4 knockdown increased necrosis but not apoptosis .
	manualset2
82128	1	397664	5	NULL	NULL	NULL	NULL	low-income areas	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , dynamic market forces will gradually reduce the quality of care in low-income areas while both access and quality of care will be even better in high-income areas .
	manualset2
82131	2	397664	5	NULL	NULL	NULL	NULL	high-income areas	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , dynamic market forces will gradually reduce the quality of care in low-income areas while both access and quality of care will be even better in high-income areas .
	manualset2
82132	1	397665	5	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , each of the nonspecifically protected mice of both the BALB/c and P/J strains developed immunity to rechallenge with viable L. major .
	manualset2
82133	2	397665	5	NULL	NULL	NULL	NULL	BALB/c and P/J strains	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , each of the nonspecifically protected mice of both the BALB/c and P/J strains developed immunity to rechallenge with viable L. major .
	manualset2
82136	3	397665	5	NULL	NULL	NULL	NULL	immunity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , each of the nonspecifically protected mice of both the BALB/c and P/J strains developed immunity to rechallenge with viable L. major .
	manualset2
82137	4	397665	5	NULL	NULL	NULL	NULL	viable L. major	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , each of the nonspecifically protected mice of both the BALB/c and P/J strains developed immunity to rechallenge with viable L. major .
	manualset2
82138	2	397666	5	NULL	NULL	NULL	NULL	Fxr-null mice	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , experiments with Fxr-null mice suggest that cholesterol feeding can down-regulate ASBT expression through a pathway independent of FXR .
	manualset2
82140	1	397666	5	NULL	NULL	0	NULL	experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , experiments with Fxr-null mice suggest that cholesterol feeding can down-regulate ASBT expression through a pathway independent of FXR .
	manualset2
82141	3	397666	5	NULL	NULL	NULL	NULL	cholesterol feeding	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , experiments with Fxr-null mice suggest that cholesterol feeding can down-regulate ASBT expression through a pathway independent of FXR .
	manualset2
82142	4	397666	5	NULL	NULL	NULL	NULL	ASBT expression	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , experiments with Fxr-null mice suggest that cholesterol feeding can down-regulate ASBT expression through a pathway independent of FXR .
	manualset2
82144	5	397666	5	NULL	NULL	NULL	NULL	pathway independent of FXR	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , experiments with Fxr-null mice suggest that cholesterol feeding can down-regulate ASBT expression through a pathway independent of FXR .
	manualset2
82146	1	397667	5	NULL	NULL	NULL	NULL	low-energy conformations ( LECs )	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , from superpositions of low-energy conformations ( LECs ) of 1 , 2 , and ( S ) -6 al , it was concluded that a common binding conformation ( LEC II ; Figure 10B ) may exist and that differences in binding to the SU receptor and in the mechanism of insulin release between repaglinide and the two SUs may be due to specific hydrophobic differences .
	manualset2
82150	3	397667	5	NULL	NULL	NULL	NULL	LEC II	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , from superpositions of low-energy conformations ( LECs ) of 1 , 2 , and ( S ) -6 al , it was concluded that a common binding conformation ( LEC II ; Figure 10B ) may exist and that differences in binding to the SU receptor and in the mechanism of insulin release between repaglinide and the two SUs may be due to specific hydrophobic differences .
	manualset2
82151	4	397667	5	NULL	NULL	NULL	NULL	SU receptor	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , from superpositions of low-energy conformations ( LECs ) of 1 , 2 , and ( S ) -6 al , it was concluded that a common binding conformation ( LEC II ; Figure 10B ) may exist and that differences in binding to the SU receptor and in the mechanism of insulin release between repaglinide and the two SUs may be due to specific hydrophobic differences .
	manualset2
82153	5	397667	5	NULL	NULL	NULL	NULL	mechanism of insulin release	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , from superpositions of low-energy conformations ( LECs ) of 1 , 2 , and ( S ) -6 al , it was concluded that a common binding conformation ( LEC II ; Figure 10B ) may exist and that differences in binding to the SU receptor and in the mechanism of insulin release between repaglinide and the two SUs may be due to specific hydrophobic differences .
	manualset2
82154	6	397667	5	NULL	NULL	NULL	NULL	repaglinide	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , from superpositions of low-energy conformations ( LECs ) of 1 , 2 , and ( S ) -6 al , it was concluded that a common binding conformation ( LEC II ; Figure 10B ) may exist and that differences in binding to the SU receptor and in the mechanism of insulin release between repaglinide and the two SUs may be due to specific hydrophobic differences .
	manualset2
82155	7	397667	5	NULL	NULL	NULL	NULL	SUs	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , from superpositions of low-energy conformations ( LECs ) of 1 , 2 , and ( S ) -6 al , it was concluded that a common binding conformation ( LEC II ; Figure 10B ) may exist and that differences in binding to the SU receptor and in the mechanism of insulin release between repaglinide and the two SUs may be due to specific hydrophobic differences .
	manualset2
82551	2	397667	5	NULL	NULL	0	NULL	common binding conformation	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , from superpositions of low-energy conformations ( LECs ) of 1 , 2 , and ( S ) -6 al , it was concluded that a common binding conformation ( LEC II ; Figure 10B ) may exist and that differences in binding to the SU receptor and in the mechanism of insulin release between repaglinide and the two SUs may be due to specific hydrophobic differences .
	manualset2
82552	8	397667	5	NULL	NULL	0	NULL	hydrophobic differences	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , from superpositions of low-energy conformations ( LECs ) of 1 , 2 , and ( S ) -6 al , it was concluded that a common binding conformation ( LEC II ; Figure 10B ) may exist and that differences in binding to the SU receptor and in the mechanism of insulin release between repaglinide and the two SUs may be due to specific hydrophobic differences .
	manualset2
82156	1	397668	5	NULL	NULL	NULL	NULL	immature B cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , immature B cells have been widely shown to be hypersensitive to tolerance induction .
	manualset2
82157	2	397668	5	NULL	NULL	NULL	NULL	tolerance induction	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , immature B cells have been widely shown to be hypersensitive to tolerance induction .
	manualset2
82159	3	397669	5	NULL	NULL	NULL	NULL	rehabilitation programs	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Round table discussion : the psychological aspect of rehabilitation programs ) .
	manualset2
82553	1	397669	5	NULL	NULL	NULL	NULL	Round table discussion	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Round table discussion : the psychological aspect of rehabilitation programs ) .
	manualset2
82554	2	397669	5	NULL	NULL	0	NULL	psychological aspect	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Round table discussion : the psychological aspect of rehabilitation programs ) .
	manualset2
82160	1	397670	5	NULL	NULL	NULL	NULL	intact cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in intact cells addition of 1 mM selenate stimulated tyrosyl phosphorylation of 210 - , 170 - , 120 - , 95 - , 70 - , and 60-kDa proteins but failed to stimulate insulin receptor kinase activity , suggesting that selenate stimulated other tyrosine kinase .
	manualset2
82161	2	397670	5	NULL	NULL	NULL	NULL	addition	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in intact cells addition of 1 mM selenate stimulated tyrosyl phosphorylation of 210 - , 170 - , 120 - , 95 - , 70 - , and 60-kDa proteins but failed to stimulate insulin receptor kinase activity , suggesting that selenate stimulated other tyrosine kinase .
	manualset2
82162	3	397670	5	NULL	NULL	NULL	NULL	1 mM selenate	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in intact cells addition of 1 mM selenate stimulated tyrosyl phosphorylation of 210 - , 170 - , 120 - , 95 - , 70 - , and 60-kDa proteins but failed to stimulate insulin receptor kinase activity , suggesting that selenate stimulated other tyrosine kinase .
	manualset2
82163	4	397670	5	NULL	NULL	NULL	NULL	tyrosyl phosphorylation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in intact cells addition of 1 mM selenate stimulated tyrosyl phosphorylation of 210 - , 170 - , 120 - , 95 - , 70 - , and 60-kDa proteins but failed to stimulate insulin receptor kinase activity , suggesting that selenate stimulated other tyrosine kinase .
	manualset2
82165	6	397670	5	NULL	NULL	NULL	NULL	stimulate	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in intact cells addition of 1 mM selenate stimulated tyrosyl phosphorylation of 210 - , 170 - , 120 - , 95 - , 70 - , and 60-kDa proteins but failed to stimulate insulin receptor kinase activity , suggesting that selenate stimulated other tyrosine kinase .
	manualset2
82166	7	397670	5	NULL	NULL	NULL	NULL	insulin receptor kinase activity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in intact cells addition of 1 mM selenate stimulated tyrosyl phosphorylation of 210 - , 170 - , 120 - , 95 - , 70 - , and 60-kDa proteins but failed to stimulate insulin receptor kinase activity , suggesting that selenate stimulated other tyrosine kinase .
	manualset2
82170	8	397670	5	NULL	NULL	NULL	NULL	selenate	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in intact cells addition of 1 mM selenate stimulated tyrosyl phosphorylation of 210 - , 170 - , 120 - , 95 - , 70 - , and 60-kDa proteins but failed to stimulate insulin receptor kinase activity , suggesting that selenate stimulated other tyrosine kinase .
	manualset2
82171	9	397670	5	NULL	NULL	NULL	NULL	tyrosine kinase	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in intact cells addition of 1 mM selenate stimulated tyrosyl phosphorylation of 210 - , 170 - , 120 - , 95 - , 70 - , and 60-kDa proteins but failed to stimulate insulin receptor kinase activity , suggesting that selenate stimulated other tyrosine kinase .
	manualset2
82535	5	397670	5	NULL	NULL	NULL	NULL	210 - , 170 - , 120 - , 95 - , 70 - , and 60-kDa proteins	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in intact cells addition of 1 mM selenate stimulated tyrosyl phosphorylation of 210 - , 170 - , 120 - , 95 - , 70 - , and 60-kDa proteins but failed to stimulate insulin receptor kinase activity , suggesting that selenate stimulated other tyrosine kinase .
	manualset2
82173	1	397671	5	NULL	NULL	0	NULL	media	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , in media with physiological concentrations of glucose or pyruvate , A2E significantly inhibited phagocytosis .
	manualset2
82174	2	397671	5	NULL	NULL	NULL	NULL	physiological concentrations	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in media with physiological concentrations of glucose or pyruvate , A2E significantly inhibited phagocytosis .
	manualset2
82175	3	397671	5	NULL	NULL	NULL	NULL	glucose	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in media with physiological concentrations of glucose or pyruvate , A2E significantly inhibited phagocytosis .
	manualset2
82176	4	397671	5	NULL	NULL	NULL	NULL	pyruvate	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in media with physiological concentrations of glucose or pyruvate , A2E significantly inhibited phagocytosis .
	manualset2
82177	5	397671	5	NULL	NULL	0	NULL	A2E	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , in media with physiological concentrations of glucose or pyruvate , A2E significantly inhibited phagocytosis .
	manualset2
82178	6	397671	5	NULL	NULL	0	NULL	phagocytosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , in media with physiological concentrations of glucose or pyruvate , A2E significantly inhibited phagocytosis .
	manualset2
82179	1	397672	5	NULL	NULL	NULL	NULL	platelets and endothelial cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in platelets and endothelial cells , the enzyme activity was localized in the membrane fraction and was distinct from cytosolic glutathione-S-transferases .
	manualset2
82181	2	397672	5	NULL	NULL	NULL	NULL	enzyme activity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in platelets and endothelial cells , the enzyme activity was localized in the membrane fraction and was distinct from cytosolic glutathione-S-transferases .
	manualset2
82183	3	397672	5	NULL	NULL	NULL	NULL	membrane fraction	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in platelets and endothelial cells , the enzyme activity was localized in the membrane fraction and was distinct from cytosolic glutathione-S-transferases .
	manualset2
82186	4	397672	5	NULL	NULL	NULL	NULL	cytosolic glutathione-S-transferases	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in platelets and endothelial cells , the enzyme activity was localized in the membrane fraction and was distinct from cytosolic glutathione-S-transferases .
	manualset2
82187	1	397673	5	NULL	NULL	0	NULL	response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , in response to DNA damage , p53 and hnRNP K are recruited to the promoters of p53-responsive genes in a mutually dependent manner .
	manualset2
82188	2	397673	5	NULL	NULL	NULL	NULL	DNA damage	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in response to DNA damage , p53 and hnRNP K are recruited to the promoters of p53-responsive genes in a mutually dependent manner .
	manualset2
82190	4	397673	5	NULL	NULL	0	NULL	p53	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , in response to DNA damage , p53 and hnRNP K are recruited to the promoters of p53-responsive genes in a mutually dependent manner .
	manualset2
82191	5	397673	5	NULL	NULL	0	NULL	hnRNP K	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , in response to DNA damage , p53 and hnRNP K are recruited to the promoters of p53-responsive genes in a mutually dependent manner .
	manualset2
82192	6	397673	5	NULL	NULL	NULL	NULL	promoters of p53-responsive genes	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in response to DNA damage , p53 and hnRNP K are recruited to the promoters of p53-responsive genes in a mutually dependent manner .
	manualset2
82195	1	397674	5	NULL	NULL	NULL	NULL	S447X polymorphism	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in the case of the S447X polymorphism , 447Ter carriers had a lower postprandial response for small TRL-RP , large TRL-B48 , and small TRL-RP .
	manualset2
82197	2	397674	5	NULL	NULL	NULL	NULL	447Ter carriers	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in the case of the S447X polymorphism , 447Ter carriers had a lower postprandial response for small TRL-RP , large TRL-B48 , and small TRL-RP .
	manualset2
82198	3	397674	5	NULL	NULL	NULL	NULL	postprandial response	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in the case of the S447X polymorphism , 447Ter carriers had a lower postprandial response for small TRL-RP , large TRL-B48 , and small TRL-RP .
	manualset2
82200	4	397674	5	NULL	NULL	NULL	NULL	TRL-RP	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in the case of the S447X polymorphism , 447Ter carriers had a lower postprandial response for small TRL-RP , large TRL-B48 , and small TRL-RP .
	manualset2
82201	5	397674	5	NULL	NULL	NULL	NULL	TRL-B48	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in the case of the S447X polymorphism , 447Ter carriers had a lower postprandial response for small TRL-RP , large TRL-B48 , and small TRL-RP .
	manualset2
82202	6	397674	5	NULL	NULL	NULL	NULL	TRL-RP	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in the case of the S447X polymorphism , 447Ter carriers had a lower postprandial response for small TRL-RP , large TRL-B48 , and small TRL-RP .
	manualset2
82203	1	397675	5	NULL	NULL	NULL	NULL	vitamin E	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in the group treated with vitamin E , distinct recovery of EEG potentials at three hours after recirculation was apparent .
	manualset2
82204	2	397675	5	NULL	NULL	0	NULL	EEG	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , in the group treated with vitamin E , distinct recovery of EEG potentials at three hours after recirculation was apparent .
	manualset2
82205	3	397675	5	NULL	NULL	0	NULL	potentials	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , in the group treated with vitamin E , distinct recovery of EEG potentials at three hours after recirculation was apparent .
	manualset2
82206	4	397675	5	NULL	NULL	NULL	NULL	three hours	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in the group treated with vitamin E , distinct recovery of EEG potentials at three hours after recirculation was apparent .
	manualset2
82207	5	397675	5	NULL	NULL	0	NULL	recirculation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , in the group treated with vitamin E , distinct recovery of EEG potentials at three hours after recirculation was apparent .
	manualset2
82208	1	397676	5	NULL	NULL	NULL	NULL	p53 gene	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in the light of previous findings that the p53 gene in most UNPCs is in the wild-type configuration , mechanisms other than mutation may be responsible for stabilisation of the p53 protein in UNPCs .
	manualset2
82210	2	397676	5	NULL	NULL	NULL	NULL	UNPCs	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in the light of previous findings that the p53 gene in most UNPCs is in the wild-type configuration , mechanisms other than mutation may be responsible for stabilisation of the p53 protein in UNPCs .
	manualset2
82212	3	397676	5	NULL	NULL	NULL	NULL	mechanisms	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in the light of previous findings that the p53 gene in most UNPCs is in the wild-type configuration , mechanisms other than mutation may be responsible for stabilisation of the p53 protein in UNPCs .
	manualset2
82213	4	397676	5	NULL	NULL	NULL	NULL	mutation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in the light of previous findings that the p53 gene in most UNPCs is in the wild-type configuration , mechanisms other than mutation may be responsible for stabilisation of the p53 protein in UNPCs .
	manualset2
82214	5	397676	5	NULL	NULL	NULL	NULL	stabilisation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in the light of previous findings that the p53 gene in most UNPCs is in the wild-type configuration , mechanisms other than mutation may be responsible for stabilisation of the p53 protein in UNPCs .
	manualset2
82215	6	397676	5	NULL	NULL	NULL	NULL	p53 protein	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in the light of previous findings that the p53 gene in most UNPCs is in the wild-type configuration , mechanisms other than mutation may be responsible for stabilisation of the p53 protein in UNPCs .
	manualset2
82217	7	397676	5	NULL	NULL	NULL	NULL	UNPCs	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , in the light of previous findings that the p53 gene in most UNPCs is in the wild-type configuration , mechanisms other than mutation may be responsible for stabilisation of the p53 protein in UNPCs .
	manualset2
82218	1	397677	5	NULL	NULL	NULL	NULL	apple juice	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , it was not possible to acidify apple juice to a pH of 2.0 to completely inhibit enzymatic browning .
	manualset2
82220	2	397677	5	NULL	NULL	NULL	NULL	pH of 2.0	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , it was not possible to acidify apple juice to a pH of 2.0 to completely inhibit enzymatic browning .
	manualset2
82223	3	397677	5	NULL	NULL	NULL	NULL	enzymatic browning	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , it was not possible to acidify apple juice to a pH of 2.0 to completely inhibit enzymatic browning .
	manualset2
82224	1	397678	5	NULL	NULL	NULL	NULL	mRNA 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , mRNA and protein levels of E-cadherin ( CDH1 ) were decreased in siRNA microinjected blastocysts .
	manualset2
82226	3	397678	5	NULL	NULL	NULL	NULL	E-cadherin ( CDH1 )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , mRNA and protein levels of E-cadherin ( CDH1 ) were decreased in siRNA microinjected blastocysts .
	manualset2
82228	4	397678	5	NULL	NULL	NULL	NULL	siRNA microinjected blastocysts	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , mRNA and protein levels of E-cadherin ( CDH1 ) were decreased in siRNA microinjected blastocysts .
	manualset2
82558	2	397678	5	NULL	NULL	NULL	NULL	protein 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , mRNA and protein levels of E-cadherin ( CDH1 ) were decreased in siRNA microinjected blastocysts .
	manualset2
82230	1	397679	5	NULL	NULL	0	NULL	Rubiaceae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Rubiaceae ) is an important component of the ayurvedic system of medicine .
	manualset2
82231	2	397679	5	NULL	NULL	NULL	NULL	important component	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Rubiaceae ) is an important component of the ayurvedic system of medicine .
	manualset2
82232	3	397679	5	NULL	NULL	NULL	NULL	ayurvedic system of medicine	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Rubiaceae ) is an important component of the ayurvedic system of medicine .
	manualset2
82236	2	397680	5	NULL	NULL	NULL	NULL	agar	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , minimal inhibitory concentration and minimal lethal concentration for different bacterial species in presence of agar were significantly lower than those observed in presence of tween 80 or ethanol .
	manualset2
82237	3	397680	5	NULL	NULL	NULL	NULL	tween 80	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , minimal inhibitory concentration and minimal lethal concentration for different bacterial species in presence of agar were significantly lower than those observed in presence of tween 80 or ethanol .
	manualset2
82238	4	397680	5	NULL	NULL	NULL	NULL	ethanol	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , minimal inhibitory concentration and minimal lethal concentration for different bacterial species in presence of agar were significantly lower than those observed in presence of tween 80 or ethanol .
	manualset2
82239	1	397680	5	NULL	NULL	NULL	NULL	bacterial species	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , minimal inhibitory concentration and minimal lethal concentration for different bacterial species in presence of agar were significantly lower than those observed in presence of tween 80 or ethanol .
	manualset2
82240	1	397681	5	NULL	NULL	NULL	NULL	mutant yeast cells	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , mutant yeast cells show increased susceptibility to a nitrosative challenge , whereas their resistance to oxidative stress is unimpaired .
	manualset2
82242	2	397681	5	NULL	NULL	NULL	NULL	increased susceptibility	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , mutant yeast cells show increased susceptibility to a nitrosative challenge , whereas their resistance to oxidative stress is unimpaired .
	manualset2
82243	3	397681	5	NULL	NULL	NULL	NULL	nitrosative challenge	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , mutant yeast cells show increased susceptibility to a nitrosative challenge , whereas their resistance to oxidative stress is unimpaired .
	manualset2
82244	4	397681	5	NULL	NULL	NULL	NULL	resistance to oxidative stress	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , mutant yeast cells show increased susceptibility to a nitrosative challenge , whereas their resistance to oxidative stress is unimpaired .
	manualset2
82246	1	397682	5	NULL	NULL	0	NULL	mutation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , mutation at the tyrosine phosphorylation site in the cytoplasmic domain of C-CAM1 did not obliterate C-CAM1 's growth suppression function , suggesting that tyrosine phosphorylation is not involved in the signal transduction pathway leading to cell growth suppression .
	manualset2
82247	2	397682	5	NULL	NULL	NULL	NULL	tyrosine phosphorylation site	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , mutation at the tyrosine phosphorylation site in the cytoplasmic domain of C-CAM1 did not obliterate C-CAM1 's growth suppression function , suggesting that tyrosine phosphorylation is not involved in the signal transduction pathway leading to cell growth suppression .
	manualset2
82250	3	397682	5	NULL	NULL	NULL	NULL	cytoplasmic domain	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , mutation at the tyrosine phosphorylation site in the cytoplasmic domain of C-CAM1 did not obliterate C-CAM1 's growth suppression function , suggesting that tyrosine phosphorylation is not involved in the signal transduction pathway leading to cell growth suppression .
	manualset2
82251	4	397682	5	NULL	NULL	NULL	NULL	C-CAM1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , mutation at the tyrosine phosphorylation site in the cytoplasmic domain of C-CAM1 did not obliterate C-CAM1 's growth suppression function , suggesting that tyrosine phosphorylation is not involved in the signal transduction pathway leading to cell growth suppression .
	manualset2
82252	5	397682	5	NULL	NULL	NULL	NULL	C-CAM1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , mutation at the tyrosine phosphorylation site in the cytoplasmic domain of C-CAM1 did not obliterate C-CAM1 's growth suppression function , suggesting that tyrosine phosphorylation is not involved in the signal transduction pathway leading to cell growth suppression .
	manualset2
82253	6	397682	5	NULL	NULL	NULL	NULL	growth suppression function	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , mutation at the tyrosine phosphorylation site in the cytoplasmic domain of C-CAM1 did not obliterate C-CAM1 's growth suppression function , suggesting that tyrosine phosphorylation is not involved in the signal transduction pathway leading to cell growth suppression .
	manualset2
82256	7	397682	5	NULL	NULL	NULL	NULL	tyrosine phosphorylation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , mutation at the tyrosine phosphorylation site in the cytoplasmic domain of C-CAM1 did not obliterate C-CAM1 's growth suppression function , suggesting that tyrosine phosphorylation is not involved in the signal transduction pathway leading to cell growth suppression .
	manualset2
82258	8	397682	5	NULL	NULL	NULL	NULL	signal transduction pathway	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , mutation at the tyrosine phosphorylation site in the cytoplasmic domain of C-CAM1 did not obliterate C-CAM1 's growth suppression function , suggesting that tyrosine phosphorylation is not involved in the signal transduction pathway leading to cell growth suppression .
	manualset2
82259	9	397682	5	NULL	NULL	NULL	NULL	cell growth suppression	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , mutation at the tyrosine phosphorylation site in the cytoplasmic domain of C-CAM1 did not obliterate C-CAM1 's growth suppression function , suggesting that tyrosine phosphorylation is not involved in the signal transduction pathway leading to cell growth suppression .
	manualset2
82263	1	397683	5	NULL	NULL	NULL	NULL	nicotine	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , nicotine modulates cognitive networks involved in attention and learning/memory .
	manualset2
82264	2	397683	5	NULL	NULL	NULL	NULL	cognitive networks	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , nicotine modulates cognitive networks involved in attention and learning/memory .
	manualset2
82266	3	397683	5	NULL	NULL	NULL	NULL	attention	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , nicotine modulates cognitive networks involved in attention and learning/memory .
	manualset2
82267	4	397683	5	NULL	NULL	NULL	NULL	learning/memory	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , nicotine modulates cognitive networks involved in attention and learning/memory .
	manualset2
82269	1	397684	5	NULL	NULL	NULL	NULL	time	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , nuclear grade was associated with time to recurrence ( P = 0.004 ) in patients who underwent complete surgical resection ( n = 159 ) .
	manualset2
82270	3	397684	5	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , nuclear grade was associated with time to recurrence ( P = 0.004 ) in patients who underwent complete surgical resection ( n = 159 ) .
	manualset2
82271	2	397684	5	NULL	NULL	NULL	NULL	recurrence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , nuclear grade was associated with time to recurrence ( P = 0.004 ) in patients who underwent complete surgical resection ( n = 159 ) .
	manualset2
82272	4	397684	5	NULL	NULL	NULL	NULL	surgical resection	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , nuclear grade was associated with time to recurrence ( P = 0.004 ) in patients who underwent complete surgical resection ( n = 159 ) .
	manualset2
82273	1	397685	5	NULL	NULL	NULL	NULL	IAP elements	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , one of the IAP elements ( belonging to the LS1 subfamily ) is specifically hypomethylated in the DNA of the immunogenic cells .
	manualset2
82275	2	397685	5	NULL	NULL	NULL	NULL	LS1 subfamily	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , one of the IAP elements ( belonging to the LS1 subfamily ) is specifically hypomethylated in the DNA of the immunogenic cells .
	manualset2
82278	3	397685	5	NULL	NULL	NULL	NULL	DNA	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , one of the IAP elements ( belonging to the LS1 subfamily ) is specifically hypomethylated in the DNA of the immunogenic cells .
	manualset2
82559	4	397685	5	NULL	NULL	0	NULL	immunogenic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , one of the IAP elements ( belonging to the LS1 subfamily ) is specifically hypomethylated in the DNA of the immunogenic cells .
	manualset2
82280	1	397686	5	NULL	NULL	0	NULL	oocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , oocytes cultured with FSH maintained trans-zonal projections of cumulus cells .
	manualset2
82281	2	397686	5	NULL	NULL	0	NULL	FSH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , oocytes cultured with FSH maintained trans-zonal projections of cumulus cells .
	manualset2
82282	3	397686	5	NULL	NULL	NULL	NULL	trans-zonal projections	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , oocytes cultured with FSH maintained trans-zonal projections of cumulus cells .
	manualset2
82283	4	397686	5	NULL	NULL	NULL	NULL	cumulus cell	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , oocytes cultured with FSH maintained trans-zonal projections of cumulus cells .
	manualset2
82285	1	397687	5	NULL	NULL	NULL	NULL	oral administration	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , oral administration of loratadine at a dose of 10 mg/kg for 7 days also significantly inhibited the histamine-induced scratching behavior in the same animals .
	manualset2
82286	2	397687	5	NULL	NULL	0	NULL	loratadine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , oral administration of loratadine at a dose of 10 mg/kg for 7 days also significantly inhibited the histamine-induced scratching behavior in the same animals .
	manualset2
82287	3	397687	5	NULL	NULL	0	NULL	10 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , oral administration of loratadine at a dose of 10 mg/kg for 7 days also significantly inhibited the histamine-induced scratching behavior in the same animals .
	manualset2
82288	4	397687	5	NULL	NULL	NULL	NULL	7 days	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , oral administration of loratadine at a dose of 10 mg/kg for 7 days also significantly inhibited the histamine-induced scratching behavior in the same animals .
	manualset2
82289	5	397687	5	NULL	NULL	NULL	NULL	histamine-induced scratching behavior	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , oral administration of loratadine at a dose of 10 mg/kg for 7 days also significantly inhibited the histamine-induced scratching behavior in the same animals .
	manualset2
82291	6	397687	5	NULL	NULL	NULL	NULL	animals	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , oral administration of loratadine at a dose of 10 mg/kg for 7 days also significantly inhibited the histamine-induced scratching behavior in the same animals .
	manualset2
82292	1	397688	5	NULL	NULL	0	NULL	pH	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , pH changes correlated with the 3NP-induced inhibition of succinate dehydrogenase and preceded striatum lesions .
	manualset2
82293	2	397688	5	NULL	NULL	NULL	NULL	3NP	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , pH changes correlated with the 3NP-induced inhibition of succinate dehydrogenase and preceded striatum lesions .
	manualset2
82294	3	397688	5	NULL	NULL	NULL	NULL	3NP-induced inhibition	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , pH changes correlated with the 3NP-induced inhibition of succinate dehydrogenase and preceded striatum lesions .
	manualset2
82295	4	397688	5	NULL	NULL	0	NULL	succinate dehydrogenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , pH changes correlated with the 3NP-induced inhibition of succinate dehydrogenase and preceded striatum lesions .
	manualset2
82296	5	397688	5	NULL	NULL	NULL	NULL	striatum lesions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , pH changes correlated with the 3NP-induced inhibition of succinate dehydrogenase and preceded striatum lesions .
	manualset2
82298	2	397689	5	NULL	NULL	NULL	NULL	L1210/CPA cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , pretreatment of L1210/CPA cells with the ADH inhibitor , diethyl aminobenzaldehyde ( DEAB ) , resulted in potentiation of the SDA response .
	manualset2
82299	3	397689	5	NULL	NULL	NULL	NULL	ADH inhibitor	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , pretreatment of L1210/CPA cells with the ADH inhibitor , diethyl aminobenzaldehyde ( DEAB ) , resulted in potentiation of the SDA response .
	manualset2
82300	4	397689	5	NULL	NULL	NULL	NULL	diethyl aminobenzaldehyde  ( DEAB )	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , pretreatment of L1210/CPA cells with the ADH inhibitor , diethyl aminobenzaldehyde ( DEAB ) , resulted in potentiation of the SDA response .
	manualset2
82302	5	397689	5	NULL	NULL	NULL	NULL	potentiation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , pretreatment of L1210/CPA cells with the ADH inhibitor , diethyl aminobenzaldehyde ( DEAB ) , resulted in potentiation of the SDA response .
	manualset2
82303	6	397689	5	NULL	NULL	NULL	NULL	SDA response	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , pretreatment of L1210/CPA cells with the ADH inhibitor , diethyl aminobenzaldehyde ( DEAB ) , resulted in potentiation of the SDA response .
	manualset2
82537	1	397689	5	NULL	NULL	0	NULL	pretreatment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , pretreatment of L1210/CPA cells with the ADH inhibitor , diethyl aminobenzaldehyde ( DEAB ) , resulted in potentiation of the SDA response .
	manualset2
82305	1	397690	5	NULL	NULL	NULL	NULL	qualitative examination	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , qualitative examination of the recognition trial revealed the presence of `` atypical recognition errors '' that were endorsed with significantly higher frequency by the suspect effort patients .
	manualset2
82306	4	397690	5	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , qualitative examination of the recognition trial revealed the presence of `` atypical recognition errors '' that were endorsed with significantly higher frequency by the suspect effort patients .
	manualset2
82307	2	397690	5	NULL	NULL	NULL	NULL	recognition trial	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , qualitative examination of the recognition trial revealed the presence of `` atypical recognition errors '' that were endorsed with significantly higher frequency by the suspect effort patients .
	manualset2
82309	1	397691	5	NULL	NULL	0	NULL	quercetin	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , quercetin conjugation by different in vitro models from corresponding origins may differ significantly .
	manualset2
82310	2	397691	5	NULL	NULL	0	NULL	conjugation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , quercetin conjugation by different in vitro models from corresponding origins may differ significantly .
	manualset2
82311	1	397692	5	NULL	NULL	0	NULL	dieldrin	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , regardless of whether dieldrin was present or not , removal of vanadate 24 h before fixation of the colonies caused a slight decrease in the transformation frequency .
	manualset2
82312	2	397692	5	NULL	NULL	NULL	NULL	vanadate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , regardless of whether dieldrin was present or not , removal of vanadate 24 h before fixation of the colonies caused a slight decrease in the transformation frequency .
	manualset2
82313	3	397692	5	NULL	NULL	NULL	NULL	24 h	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , regardless of whether dieldrin was present or not , removal of vanadate 24 h before fixation of the colonies caused a slight decrease in the transformation frequency .
	manualset2
82314	4	397692	5	NULL	NULL	0	NULL	fixation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , regardless of whether dieldrin was present or not , removal of vanadate 24 h before fixation of the colonies caused a slight decrease in the transformation frequency .
	manualset2
82315	5	397692	5	NULL	NULL	0	NULL	colonies	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , regardless of whether dieldrin was present or not , removal of vanadate 24 h before fixation of the colonies caused a slight decrease in the transformation frequency .
	manualset2
82316	6	397692	5	NULL	NULL	0	NULL	transformation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , regardless of whether dieldrin was present or not , removal of vanadate 24 h before fixation of the colonies caused a slight decrease in the transformation frequency .
	manualset2
82317	1	397693	5	NULL	NULL	NULL	NULL	 management attention	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , results to date , suggest that management attention must expand from its historical focus on infra-structure provision to incorporate diffuse sources of faecal indicator loading which present a new set of management and modelling challenges .
	manualset2
82527	2	397693	5	NULL	NULL	0	NULL	focus	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , results to date , suggest that management attention must expand from its historical focus on infra-structure provision to incorporate diffuse sources of faecal indicator loading which present a new set of management and modelling challenges .
	manualset2
82528	3	397693	5	NULL	NULL	NULL	NULL	infra-structure provision	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , results to date , suggest that management attention must expand from its historical focus on infra-structure provision to incorporate diffuse sources of faecal indicator loading which present a new set of management and modelling challenges .
	manualset2
82530	4	397693	5	NULL	NULL	NULL	NULL	challenges	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , results to date , suggest that management attention must expand from its historical focus on infra-structure provision to incorporate diffuse sources of faecal indicator loading which present a new set of management and modelling challenges .
	manualset2
82318	1	397694	5	NULL	NULL	NULL	NULL	sequence	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , some sequence similarities in the 5 ' - flanking region are found between the corticotropin/beta-lipotropin precursor gene and the mouse alpha-globin and beta-globin genes , all of which are negatively regulated by glucocorticoids .
	manualset2
82319	3	397694	5	NULL	NULL	NULL	NULL	corticotropin/beta-lipotropin precursor	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , some sequence similarities in the 5 ' - flanking region are found between the corticotropin/beta-lipotropin precursor gene and the mouse alpha-globin and beta-globin genes , all of which are negatively regulated by glucocorticoids .
	manualset2
82320	4	397694	5	NULL	NULL	NULL	NULL	mouse	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , some sequence similarities in the 5 ' - flanking region are found between the corticotropin/beta-lipotropin precursor gene and the mouse alpha-globin and beta-globin genes , all of which are negatively regulated by glucocorticoids .
	manualset2
82321	2	397694	5	NULL	NULL	NULL	NULL	5 ' - flanking region	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , some sequence similarities in the 5 ' - flanking region are found between the corticotropin/beta-lipotropin precursor gene and the mouse alpha-globin and beta-globin genes , all of which are negatively regulated by glucocorticoids .
	manualset2
82322	6	397694	5	NULL	NULL	NULL	NULL	beta-globin	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , some sequence similarities in the 5 ' - flanking region are found between the corticotropin/beta-lipotropin precursor gene and the mouse alpha-globin and beta-globin genes , all of which are negatively regulated by glucocorticoids .
	manualset2
82324	8	397694	5	NULL	NULL	NULL	NULL	glucocorticoids	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , some sequence similarities in the 5 ' - flanking region are found between the corticotropin/beta-lipotropin precursor gene and the mouse alpha-globin and beta-globin genes , all of which are negatively regulated by glucocorticoids .
	manualset2
82325	5	397694	5	NULL	NULL	0	NULL	alpha-globin	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , some sequence similarities in the 5 ' - flanking region are found between the corticotropin/beta-lipotropin precursor gene and the mouse alpha-globin and beta-globin genes , all of which are negatively regulated by glucocorticoids .
	manualset2
82326	1	397695	5	NULL	NULL	0	NULL	behavioral acquisition	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , studies of blocking show that behavioral acquisition in response to one component can be hindered or blocked by pretraining with the other component .
	manualset2
82327	2	397695	5	NULL	NULL	0	NULL	response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , studies of blocking show that behavioral acquisition in response to one component can be hindered or blocked by pretraining with the other component .
	manualset2
82328	3	397695	5	NULL	NULL	0	NULL	component	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , studies of blocking show that behavioral acquisition in response to one component can be hindered or blocked by pretraining with the other component .
	manualset2
82329	4	397695	5	NULL	NULL	0	NULL	component	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , studies of blocking show that behavioral acquisition in response to one component can be hindered or blocked by pretraining with the other component .
	manualset2
82330	1	397696	5	NULL	NULL	NULL	NULL	Ad2 E1A products	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the Ad2 E1A products repress transcription activated by the immunoglobulin heavy chain enhancer in chimeric recombinants , which are either stably integrated in the genome of lymphoid cells or are present as episomes .
	manualset2
82331	2	397696	5	NULL	NULL	0	NULL	repress	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the Ad2 E1A products repress transcription activated by the immunoglobulin heavy chain enhancer in chimeric recombinants , which are either stably integrated in the genome of lymphoid cells or are present as episomes .
	manualset2
82332	3	397696	5	NULL	NULL	0	NULL	transcription	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the Ad2 E1A products repress transcription activated by the immunoglobulin heavy chain enhancer in chimeric recombinants , which are either stably integrated in the genome of lymphoid cells or are present as episomes .
	manualset2
82333	4	397696	5	NULL	NULL	NULL	NULL	immunoglobulin heavy chain enhancer	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the Ad2 E1A products repress transcription activated by the immunoglobulin heavy chain enhancer in chimeric recombinants , which are either stably integrated in the genome of lymphoid cells or are present as episomes .
	manualset2
82334	5	397696	5	NULL	NULL	0	NULL	chimeric recombinants	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the Ad2 E1A products repress transcription activated by the immunoglobulin heavy chain enhancer in chimeric recombinants , which are either stably integrated in the genome of lymphoid cells or are present as episomes .
	manualset2
82335	6	397696	5	NULL	NULL	0	NULL	genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the Ad2 E1A products repress transcription activated by the immunoglobulin heavy chain enhancer in chimeric recombinants , which are either stably integrated in the genome of lymphoid cells or are present as episomes .
	manualset2
82336	7	397696	5	NULL	NULL	0	NULL	lymphoid cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the Ad2 E1A products repress transcription activated by the immunoglobulin heavy chain enhancer in chimeric recombinants , which are either stably integrated in the genome of lymphoid cells or are present as episomes .
	manualset2
82337	8	397696	5	NULL	NULL	0	NULL	episomes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the Ad2 E1A products repress transcription activated by the immunoglobulin heavy chain enhancer in chimeric recombinants , which are either stably integrated in the genome of lymphoid cells or are present as episomes .
	manualset2
82338	1	397697	5	NULL	NULL	NULL	NULL	Danish Folkeskole	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the Danish Folkeskole , which is the Danish municipal primary and lower secondary school , uses the principle of differentiated teaching , integrating information technology , and there are no recommended textbooks in the curriculum .
	manualset2
82339	2	397697	5	NULL	NULL	0	NULL	school	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the Danish Folkeskole , which is the Danish municipal primary and lower secondary school , uses the principle of differentiated teaching , integrating information technology , and there are no recommended textbooks in the curriculum .
	manualset2
82340	3	397697	5	NULL	NULL	NULL	NULL	information technology	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the Danish Folkeskole , which is the Danish municipal primary and lower secondary school , uses the principle of differentiated teaching , integrating information technology , and there are no recommended textbooks in the curriculum .
	manualset2
82342	4	397697	5	NULL	NULL	NULL	NULL	textbooks	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the Danish Folkeskole , which is the Danish municipal primary and lower secondary school , uses the principle of differentiated teaching , integrating information technology , and there are no recommended textbooks in the curriculum .
	manualset2
82343	5	397697	5	NULL	NULL	NULL	NULL	curriculum	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the Danish Folkeskole , which is the Danish municipal primary and lower secondary school , uses the principle of differentiated teaching , integrating information technology , and there are no recommended textbooks in the curriculum .
	manualset2
82345	1	397698	5	NULL	NULL	0	NULL	Km	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the Km in whites was inversely related to plasma renin activity ( r = 0.50 ; P less than 0.005 ) .
	manualset2
82346	2	397698	5	NULL	NULL	0	NULL	whites	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the Km in whites was inversely related to plasma renin activity ( r = 0.50 ; P less than 0.005 ) .
	manualset2
82347	3	397698	5	NULL	NULL	NULL	NULL	plasma renin activity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the Km in whites was inversely related to plasma renin activity ( r = 0.50 ; P less than 0.005 ) .
	manualset2
82348	4	397698	5	NULL	NULL	NULL	NULL	r = 0.50	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the Km in whites was inversely related to plasma renin activity ( r = 0.50 ; P less than 0.005 ) .
	manualset2
82349	5	397698	5	NULL	NULL	NULL	NULL	0.005	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the Km in whites was inversely related to plasma renin activity ( r = 0.50 ; P less than 0.005 ) .
	manualset2
82350	1	397699	5	NULL	NULL	0	NULL	Ncorr value	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the Ncorr value for the copolymer ( MA ratio MAPTAC = 56 : 44 ) became much smaller by the neutralization of MA residues in the copolymer with sodium hydroxide , and comparable to those for neutral polymers such as poly ( ethylene glycol ) and poly ( N-vinylpyrrolidone ) and zwitterionic polymers such as poly ( 2-methacryloyloxyethyl phosphorylcholine ) ( PMPC ) and poly ( 3-sulfo-N , N-dimethyl-N - ( 3 ' - methacryloylaminopropyl ) propanaminium inner salt ) .
	manualset2
82351	2	397699	5	NULL	NULL	NULL	NULL	copolymer	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the Ncorr value for the copolymer ( MA ratio MAPTAC = 56 : 44 ) became much smaller by the neutralization of MA residues in the copolymer with sodium hydroxide , and comparable to those for neutral polymers such as poly ( ethylene glycol ) and poly ( N-vinylpyrrolidone ) and zwitterionic polymers such as poly ( 2-methacryloyloxyethyl phosphorylcholine ) ( PMPC ) and poly ( 3-sulfo-N , N-dimethyl-N - ( 3 ' - methacryloylaminopropyl ) propanaminium inner salt ) .
	manualset2
82353	3	397699	5	NULL	NULL	NULL	NULL	MA	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the Ncorr value for the copolymer ( MA ratio MAPTAC = 56 : 44 ) became much smaller by the neutralization of MA residues in the copolymer with sodium hydroxide , and comparable to those for neutral polymers such as poly ( ethylene glycol ) and poly ( N-vinylpyrrolidone ) and zwitterionic polymers such as poly ( 2-methacryloyloxyethyl phosphorylcholine ) ( PMPC ) and poly ( 3-sulfo-N , N-dimethyl-N - ( 3 ' - methacryloylaminopropyl ) propanaminium inner salt ) .
	manualset2
82354	4	397699	5	NULL	NULL	NULL	NULL	MAPTAC	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the Ncorr value for the copolymer ( MA ratio MAPTAC = 56 : 44 ) became much smaller by the neutralization of MA residues in the copolymer with sodium hydroxide , and comparable to those for neutral polymers such as poly ( ethylene glycol ) and poly ( N-vinylpyrrolidone ) and zwitterionic polymers such as poly ( 2-methacryloyloxyethyl phosphorylcholine ) ( PMPC ) and poly ( 3-sulfo-N , N-dimethyl-N - ( 3 ' - methacryloylaminopropyl ) propanaminium inner salt ) .
	manualset2
82355	5	397699	5	NULL	NULL	NULL	NULL	MA ratio MAPTAC = 56 : 44	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the Ncorr value for the copolymer ( MA ratio MAPTAC = 56 : 44 ) became much smaller by the neutralization of MA residues in the copolymer with sodium hydroxide , and comparable to those for neutral polymers such as poly ( ethylene glycol ) and poly ( N-vinylpyrrolidone ) and zwitterionic polymers such as poly ( 2-methacryloyloxyethyl phosphorylcholine ) ( PMPC ) and poly ( 3-sulfo-N , N-dimethyl-N - ( 3 ' - methacryloylaminopropyl ) propanaminium inner salt ) .
	manualset2
82356	6	397699	5	NULL	NULL	0	NULL	neutralization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the Ncorr value for the copolymer ( MA ratio MAPTAC = 56 : 44 ) became much smaller by the neutralization of MA residues in the copolymer with sodium hydroxide , and comparable to those for neutral polymers such as poly ( ethylene glycol ) and poly ( N-vinylpyrrolidone ) and zwitterionic polymers such as poly ( 2-methacryloyloxyethyl phosphorylcholine ) ( PMPC ) and poly ( 3-sulfo-N , N-dimethyl-N - ( 3 ' - methacryloylaminopropyl ) propanaminium inner salt ) .
	manualset2
82357	7	397699	5	NULL	NULL	NULL	NULL	MA	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the Ncorr value for the copolymer ( MA ratio MAPTAC = 56 : 44 ) became much smaller by the neutralization of MA residues in the copolymer with sodium hydroxide , and comparable to those for neutral polymers such as poly ( ethylene glycol ) and poly ( N-vinylpyrrolidone ) and zwitterionic polymers such as poly ( 2-methacryloyloxyethyl phosphorylcholine ) ( PMPC ) and poly ( 3-sulfo-N , N-dimethyl-N - ( 3 ' - methacryloylaminopropyl ) propanaminium inner salt ) .
	manualset2
82358	8	397699	5	NULL	NULL	NULL	NULL	copolymer	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the Ncorr value for the copolymer ( MA ratio MAPTAC = 56 : 44 ) became much smaller by the neutralization of MA residues in the copolymer with sodium hydroxide , and comparable to those for neutral polymers such as poly ( ethylene glycol ) and poly ( N-vinylpyrrolidone ) and zwitterionic polymers such as poly ( 2-methacryloyloxyethyl phosphorylcholine ) ( PMPC ) and poly ( 3-sulfo-N , N-dimethyl-N - ( 3 ' - methacryloylaminopropyl ) propanaminium inner salt ) .
	manualset2
82359	9	397699	5	NULL	NULL	0	NULL	sodium hydroxide	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the Ncorr value for the copolymer ( MA ratio MAPTAC = 56 : 44 ) became much smaller by the neutralization of MA residues in the copolymer with sodium hydroxide , and comparable to those for neutral polymers such as poly ( ethylene glycol ) and poly ( N-vinylpyrrolidone ) and zwitterionic polymers such as poly ( 2-methacryloyloxyethyl phosphorylcholine ) ( PMPC ) and poly ( 3-sulfo-N , N-dimethyl-N - ( 3 ' - methacryloylaminopropyl ) propanaminium inner salt ) .
	manualset2
82360	10	397699	5	NULL	NULL	NULL	NULL	neutral polymers	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the Ncorr value for the copolymer ( MA ratio MAPTAC = 56 : 44 ) became much smaller by the neutralization of MA residues in the copolymer with sodium hydroxide , and comparable to those for neutral polymers such as poly ( ethylene glycol ) and poly ( N-vinylpyrrolidone ) and zwitterionic polymers such as poly ( 2-methacryloyloxyethyl phosphorylcholine ) ( PMPC ) and poly ( 3-sulfo-N , N-dimethyl-N - ( 3 ' - methacryloylaminopropyl ) propanaminium inner salt ) .
	manualset2
82361	11	397699	5	NULL	NULL	NULL	NULL	poly ( ethylene glycol )	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the Ncorr value for the copolymer ( MA ratio MAPTAC = 56 : 44 ) became much smaller by the neutralization of MA residues in the copolymer with sodium hydroxide , and comparable to those for neutral polymers such as poly ( ethylene glycol ) and poly ( N-vinylpyrrolidone ) and zwitterionic polymers such as poly ( 2-methacryloyloxyethyl phosphorylcholine ) ( PMPC ) and poly ( 3-sulfo-N , N-dimethyl-N - ( 3 ' - methacryloylaminopropyl ) propanaminium inner salt ) .
	manualset2
82362	12	397699	5	NULL	NULL	NULL	NULL	poly ( N-vinylpyrrolidone )	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the Ncorr value for the copolymer ( MA ratio MAPTAC = 56 : 44 ) became much smaller by the neutralization of MA residues in the copolymer with sodium hydroxide , and comparable to those for neutral polymers such as poly ( ethylene glycol ) and poly ( N-vinylpyrrolidone ) and zwitterionic polymers such as poly ( 2-methacryloyloxyethyl phosphorylcholine ) ( PMPC ) and poly ( 3-sulfo-N , N-dimethyl-N - ( 3 ' - methacryloylaminopropyl ) propanaminium inner salt ) .
	manualset2
82363	13	397699	5	NULL	NULL	NULL	NULL	zwitterionic polymers	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the Ncorr value for the copolymer ( MA ratio MAPTAC = 56 : 44 ) became much smaller by the neutralization of MA residues in the copolymer with sodium hydroxide , and comparable to those for neutral polymers such as poly ( ethylene glycol ) and poly ( N-vinylpyrrolidone ) and zwitterionic polymers such as poly ( 2-methacryloyloxyethyl phosphorylcholine ) ( PMPC ) and poly ( 3-sulfo-N , N-dimethyl-N - ( 3 ' - methacryloylaminopropyl ) propanaminium inner salt ) .
	manualset2
82364	14	397699	5	NULL	NULL	NULL	NULL	poly ( 2-methacryloyloxyethyl phosphorylcholine )	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the Ncorr value for the copolymer ( MA ratio MAPTAC = 56 : 44 ) became much smaller by the neutralization of MA residues in the copolymer with sodium hydroxide , and comparable to those for neutral polymers such as poly ( ethylene glycol ) and poly ( N-vinylpyrrolidone ) and zwitterionic polymers such as poly ( 2-methacryloyloxyethyl phosphorylcholine ) ( PMPC ) and poly ( 3-sulfo-N , N-dimethyl-N - ( 3 ' - methacryloylaminopropyl ) propanaminium inner salt ) .
	manualset2
82365	15	397699	5	NULL	NULL	NULL	NULL	PMPC 	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the Ncorr value for the copolymer ( MA ratio MAPTAC = 56 : 44 ) became much smaller by the neutralization of MA residues in the copolymer with sodium hydroxide , and comparable to those for neutral polymers such as poly ( ethylene glycol ) and poly ( N-vinylpyrrolidone ) and zwitterionic polymers such as poly ( 2-methacryloyloxyethyl phosphorylcholine ) ( PMPC ) and poly ( 3-sulfo-N , N-dimethyl-N - ( 3 ' - methacryloylaminopropyl ) propanaminium inner salt ) .
	manualset2
82366	16	397699	5	NULL	NULL	NULL	NULL	poly ( 3-sulfo-N , N-dimethyl-N - ( 3 ' - methacryloylaminopropyl ) propanaminium inner salt )	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the Ncorr value for the copolymer ( MA ratio MAPTAC = 56 : 44 ) became much smaller by the neutralization of MA residues in the copolymer with sodium hydroxide , and comparable to those for neutral polymers such as poly ( ethylene glycol ) and poly ( N-vinylpyrrolidone ) and zwitterionic polymers such as poly ( 2-methacryloyloxyethyl phosphorylcholine ) ( PMPC ) and poly ( 3-sulfo-N , N-dimethyl-N - ( 3 ' - methacryloylaminopropyl ) propanaminium inner salt ) .
	manualset2
82367	1	397700	5	NULL	NULL	0	NULL	QPCR assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the QPCR assay identifies how much amplifiable DNA is in a sample and thus has the potential to predict PCR success in downstream applications such as STR analysis .
	manualset2
82368	2	397700	5	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the QPCR assay identifies how much amplifiable DNA is in a sample and thus has the potential to predict PCR success in downstream applications such as STR analysis .
	manualset2
82369	3	397700	5	NULL	NULL	0	NULL	sample	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the QPCR assay identifies how much amplifiable DNA is in a sample and thus has the potential to predict PCR success in downstream applications such as STR analysis .
	manualset2
82370	4	397700	5	NULL	NULL	0	NULL	PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the QPCR assay identifies how much amplifiable DNA is in a sample and thus has the potential to predict PCR success in downstream applications such as STR analysis .
	manualset2
82371	5	397700	5	NULL	NULL	0	NULL	applications	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the QPCR assay identifies how much amplifiable DNA is in a sample and thus has the potential to predict PCR success in downstream applications such as STR analysis .
	manualset2
82372	6	397700	5	NULL	NULL	0	NULL	STR analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the QPCR assay identifies how much amplifiable DNA is in a sample and thus has the potential to predict PCR success in downstream applications such as STR analysis .
	manualset2
82373	1	397701	5	NULL	NULL	0	NULL	endothelium	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the abnormal endothelium function can be corrected by tempol treatment , but this seems to involve mechanisms partly independent of NO .
	manualset2
82374	2	397701	5	NULL	NULL	0	NULL	function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the abnormal endothelium function can be corrected by tempol treatment , but this seems to involve mechanisms partly independent of NO .
	manualset2
82375	3	397701	5	NULL	NULL	0	NULL	tempol treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the abnormal endothelium function can be corrected by tempol treatment , but this seems to involve mechanisms partly independent of NO .
	manualset2
82376	4	397701	5	NULL	NULL	0	NULL	mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the abnormal endothelium function can be corrected by tempol treatment , but this seems to involve mechanisms partly independent of NO .
	manualset2
82377	5	397701	5	NULL	NULL	NULL	NULL	NO	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the abnormal endothelium function can be corrected by tempol treatment , but this seems to involve mechanisms partly independent of NO .
	manualset2
82378	1	397702	5	NULL	NULL	NULL	NULL	aminoethylated mutant proteins	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the aminoethylated mutant proteins form isolable complexes with a transition state analog , but with compromised stabilities .
	manualset2
82379	2	397702	5	NULL	NULL	NULL	NULL	isolable complexes	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the aminoethylated mutant proteins form isolable complexes with a transition state analog , but with compromised stabilities .
	manualset2
82380	3	397702	5	NULL	NULL	NULL	NULL	transition state analog	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the aminoethylated mutant proteins form isolable complexes with a transition state analog , but with compromised stabilities .
	manualset2
82382	1	397703	5	NULL	NULL	0	NULL	mercury	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the amount of mercury released with the time kept constant was almost independent of the pumping flow rate up to 8 L/min .
	manualset2
82383	2	397703	5	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the amount of mercury released with the time kept constant was almost independent of the pumping flow rate up to 8 L/min .
	manualset2
82384	3	397703	5	NULL	NULL	0	NULL	8 L/min	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the amount of mercury released with the time kept constant was almost independent of the pumping flow rate up to 8 L/min .
	manualset2
82385	1	397704	5	NULL	NULL	0	NULL	antioxidant	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the antioxidant activity was evaluated through DPPH scavenging activity , reducing power , - carotene bleaching inhibition and TBARS formation inhibition .
	manualset2
82386	2	397704	5	NULL	NULL	0	NULL	activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the antioxidant activity was evaluated through DPPH scavenging activity , reducing power , - carotene bleaching inhibition and TBARS formation inhibition .
	manualset2
82387	3	397704	5	NULL	NULL	NULL	NULL	DPPH	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the antioxidant activity was evaluated through DPPH scavenging activity , reducing power , - carotene bleaching inhibition and TBARS formation inhibition .
	manualset2
82388	4	397704	5	NULL	NULL	NULL	NULL	scavenging activity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the antioxidant activity was evaluated through DPPH scavenging activity , reducing power , - carotene bleaching inhibition and TBARS formation inhibition .
	manualset2
82389	5	397704	5	NULL	NULL	NULL	NULL	carotene	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the antioxidant activity was evaluated through DPPH scavenging activity , reducing power , - carotene bleaching inhibition and TBARS formation inhibition .
	manualset2
82390	6	397704	5	NULL	NULL	0	NULL	inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the antioxidant activity was evaluated through DPPH scavenging activity , reducing power , - carotene bleaching inhibition and TBARS formation inhibition .
	manualset2
82391	7	397704	5	NULL	NULL	NULL	NULL	TBARS	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the antioxidant activity was evaluated through DPPH scavenging activity , reducing power , - carotene bleaching inhibition and TBARS formation inhibition .
	manualset2
82392	8	397704	5	NULL	NULL	0	NULL	formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the antioxidant activity was evaluated through DPPH scavenging activity , reducing power , - carotene bleaching inhibition and TBARS formation inhibition .
	manualset2
82393	9	397704	5	NULL	NULL	0	NULL	inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the antioxidant activity was evaluated through DPPH scavenging activity , reducing power , - carotene bleaching inhibition and TBARS formation inhibition .
	manualset2
82394	1	397705	5	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the data suggest that female-specific regulation of dsx RNA processing occurs by promoting the usage of the female splice acceptor site , rather than by repressing the usage of the alternative male-specific splice acceptor .
	manualset2
82395	2	397705	5	NULL	NULL	0	NULL	female	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the data suggest that female-specific regulation of dsx RNA processing occurs by promoting the usage of the female splice acceptor site , rather than by repressing the usage of the alternative male-specific splice acceptor .
	manualset2
82396	3	397705	5	NULL	NULL	0	NULL	regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the data suggest that female-specific regulation of dsx RNA processing occurs by promoting the usage of the female splice acceptor site , rather than by repressing the usage of the alternative male-specific splice acceptor .
	manualset2
82397	4	397705	5	NULL	NULL	0	NULL	dsx RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the data suggest that female-specific regulation of dsx RNA processing occurs by promoting the usage of the female splice acceptor site , rather than by repressing the usage of the alternative male-specific splice acceptor .
	manualset2
82398	5	397705	5	NULL	NULL	0	NULL	processing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the data suggest that female-specific regulation of dsx RNA processing occurs by promoting the usage of the female splice acceptor site , rather than by repressing the usage of the alternative male-specific splice acceptor .
	manualset2
82399	6	397705	5	NULL	NULL	0	NULL	female	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the data suggest that female-specific regulation of dsx RNA processing occurs by promoting the usage of the female splice acceptor site , rather than by repressing the usage of the alternative male-specific splice acceptor .
	manualset2
82400	7	397705	5	NULL	NULL	NULL	NULL	splice acceptor site	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the data suggest that female-specific regulation of dsx RNA processing occurs by promoting the usage of the female splice acceptor site , rather than by repressing the usage of the alternative male-specific splice acceptor .
	manualset2
82401	8	397705	5	NULL	NULL	0	NULL	male	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the data suggest that female-specific regulation of dsx RNA processing occurs by promoting the usage of the female splice acceptor site , rather than by repressing the usage of the alternative male-specific splice acceptor .
	manualset2
82402	9	397705	5	NULL	NULL	0	NULL	splice acceptor	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the data suggest that female-specific regulation of dsx RNA processing occurs by promoting the usage of the female splice acceptor site , rather than by repressing the usage of the alternative male-specific splice acceptor .
	manualset2
82403	1	397706	5	NULL	NULL	0	NULL	PD game	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the decision of which PD game type to investigate ( whether all PD games , PD-Chicken boundary games or Donor & Recipient games ) is important for discussing network reciprocity .
	manualset2
82404	2	397706	5	NULL	NULL	0	NULL	PD games	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the decision of which PD game type to investigate ( whether all PD games , PD-Chicken boundary games or Donor & Recipient games ) is important for discussing network reciprocity .
	manualset2
82405	3	397706	5	NULL	NULL	0	NULL	PD-Chicken boundary games	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the decision of which PD game type to investigate ( whether all PD games , PD-Chicken boundary games or Donor & Recipient games ) is important for discussing network reciprocity .
	manualset2
82406	4	397706	5	NULL	NULL	NULL	NULL	Donor & Recipient games	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the decision of which PD game type to investigate ( whether all PD games , PD-Chicken boundary games or Donor & Recipient games ) is important for discussing network reciprocity .
	manualset2
82407	5	397706	5	NULL	NULL	0	NULL	network	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the decision of which PD game type to investigate ( whether all PD games , PD-Chicken boundary games or Donor & Recipient games ) is important for discussing network reciprocity .
	manualset2
82408	6	397706	5	NULL	NULL	0	NULL	reciprocity	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the decision of which PD game type to investigate ( whether all PD games , PD-Chicken boundary games or Donor & Recipient games ) is important for discussing network reciprocity .
	manualset2
82409	1	397707	5	NULL	NULL	0	NULL	Sarcoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Sarcoma of the abdominal wall ruptured during labor ) .
	manualset2
82410	2	397707	5	NULL	NULL	0	NULL	abdominal wall	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Sarcoma of the abdominal wall ruptured during labor ) .
	manualset2
82411	3	397707	5	NULL	NULL	0	NULL	labor	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Sarcoma of the abdominal wall ruptured during labor ) .
	manualset2
82412	1	397708	5	NULL	NULL	0	NULL	expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the expression of adipophilin as a 37 kDa N-terminally truncated protein is higher in the gastrocnemius than in the quadriceps of C57BL/6J mice , especially after an 8-week high-fat diet .
	manualset2
82413	2	397708	5	NULL	NULL	0	NULL	adipophilin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the expression of adipophilin as a 37 kDa N-terminally truncated protein is higher in the gastrocnemius than in the quadriceps of C57BL/6J mice , especially after an 8-week high-fat diet .
	manualset2
82414	3	397708	5	NULL	NULL	0	NULL	37 kDa	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the expression of adipophilin as a 37 kDa N-terminally truncated protein is higher in the gastrocnemius than in the quadriceps of C57BL/6J mice , especially after an 8-week high-fat diet .
	manualset2
82415	4	397708	5	NULL	NULL	NULL	NULL	N-terminally truncated protein	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the expression of adipophilin as a 37 kDa N-terminally truncated protein is higher in the gastrocnemius than in the quadriceps of C57BL/6J mice , especially after an 8-week high-fat diet .
	manualset2
82416	5	397708	5	NULL	NULL	0	NULL	gastrocnemius	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the expression of adipophilin as a 37 kDa N-terminally truncated protein is higher in the gastrocnemius than in the quadriceps of C57BL/6J mice , especially after an 8-week high-fat diet .
	manualset2
82417	6	397708	5	NULL	NULL	0	NULL	quadriceps	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the expression of adipophilin as a 37 kDa N-terminally truncated protein is higher in the gastrocnemius than in the quadriceps of C57BL/6J mice , especially after an 8-week high-fat diet .
	manualset2
82418	7	397708	5	NULL	NULL	0	NULL	C57BL/6J mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the expression of adipophilin as a 37 kDa N-terminally truncated protein is higher in the gastrocnemius than in the quadriceps of C57BL/6J mice , especially after an 8-week high-fat diet .
	manualset2
82419	8	397708	5	NULL	NULL	NULL	NULL	8-week	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the expression of adipophilin as a 37 kDa N-terminally truncated protein is higher in the gastrocnemius than in the quadriceps of C57BL/6J mice , especially after an 8-week high-fat diet .
	manualset2
82420	9	397708	5	NULL	NULL	NULL	NULL	high-fat diet	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the expression of adipophilin as a 37 kDa N-terminally truncated protein is higher in the gastrocnemius than in the quadriceps of C57BL/6J mice , especially after an 8-week high-fat diet .
	manualset2
82422	1	397709	5	NULL	NULL	0	NULL	expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the expression of the different A-type cyclin genes responded differently upon a block at mid-S phase by DNA synthesis inhibitors .
	manualset2
82423	2	397709	5	NULL	NULL	NULL	NULL	A-type cyclin	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the expression of the different A-type cyclin genes responded differently upon a block at mid-S phase by DNA synthesis inhibitors .
	manualset2
82424	3	397709	5	NULL	NULL	NULL	NULL	block	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the expression of the different A-type cyclin genes responded differently upon a block at mid-S phase by DNA synthesis inhibitors .
	manualset2
82425	4	397709	5	NULL	NULL	NULL	NULL	mid-S phase	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the expression of the different A-type cyclin genes responded differently upon a block at mid-S phase by DNA synthesis inhibitors .
	manualset2
82426	5	397709	5	NULL	NULL	NULL	NULL	DNA synthesis inhibitors	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the expression of the different A-type cyclin genes responded differently upon a block at mid-S phase by DNA synthesis inhibitors .
	manualset2
82429	1	397710	5	NULL	NULL	0	NULL	experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the increased experience with reduced-intensity allogeneic progenitor cell transplantation allows offering this option to physically fit patients .
	manualset2
82430	2	397710	5	NULL	NULL	NULL	NULL	allogeneic progenitor	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the increased experience with reduced-intensity allogeneic progenitor cell transplantation allows offering this option to physically fit patients .
	manualset2
82431	3	397710	5	NULL	NULL	0	NULL	cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the increased experience with reduced-intensity allogeneic progenitor cell transplantation allows offering this option to physically fit patients .
	manualset2
82432	4	397710	5	NULL	NULL	0	NULL	transplantation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the increased experience with reduced-intensity allogeneic progenitor cell transplantation allows offering this option to physically fit patients .
	manualset2
82433	5	397710	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the increased experience with reduced-intensity allogeneic progenitor cell transplantation allows offering this option to physically fit patients .
	manualset2
82434	1	397711	5	NULL	NULL	NULL	NULL	cocaine	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the issue is somewhat unclear regarding cocaine and the place preference paradigm .
	manualset2
82435	2	397711	5	NULL	NULL	NULL	NULL	preference paradigm	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the issue is somewhat unclear regarding cocaine and the place preference paradigm .
	manualset2
82437	1	397712	5	NULL	NULL	0	NULL	survivors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the majority of survivors suffer long-term side-effects due to severe management modalities .
	manualset2
82438	2	397712	5	NULL	NULL	NULL	NULL	long-term side-effects	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the majority of survivors suffer long-term side-effects due to severe management modalities .
	manualset2
82439	1	397713	5	NULL	NULL	0	NULL	SLAM/SLAM	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the negative effect of SLAM/SLAM interactions on CD40L-induced DC activation was also detected in the presence of lipopolysaccharide ( LPS ) .
	manualset2
82440	2	397713	5	NULL	NULL	0	NULL	interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the negative effect of SLAM/SLAM interactions on CD40L-induced DC activation was also detected in the presence of lipopolysaccharide ( LPS ) .
	manualset2
82441	3	397713	5	NULL	NULL	0	NULL	CD40L	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the negative effect of SLAM/SLAM interactions on CD40L-induced DC activation was also detected in the presence of lipopolysaccharide ( LPS ) .
	manualset2
82442	4	397713	5	NULL	NULL	0	NULL	DC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the negative effect of SLAM/SLAM interactions on CD40L-induced DC activation was also detected in the presence of lipopolysaccharide ( LPS ) .
	manualset2
82443	5	397713	5	NULL	NULL	0	NULL	activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the negative effect of SLAM/SLAM interactions on CD40L-induced DC activation was also detected in the presence of lipopolysaccharide ( LPS ) .
	manualset2
82444	6	397713	5	NULL	NULL	NULL	NULL	lipopolysaccharide	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the negative effect of SLAM/SLAM interactions on CD40L-induced DC activation was also detected in the presence of lipopolysaccharide ( LPS ) .
	manualset2
82445	7	397713	5	NULL	NULL	NULL	NULL	LPS	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the negative effect of SLAM/SLAM interactions on CD40L-induced DC activation was also detected in the presence of lipopolysaccharide ( LPS ) .
	manualset2
82446	1	397714	5	NULL	NULL	0	NULL	rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the nude rat CD8 + subset contained a substantial number of OX22 - cells which were nearly absent in normal rats .
	manualset2
82447	2	397714	5	NULL	NULL	0	NULL	CD8 +	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the nude rat CD8 + subset contained a substantial number of OX22 - cells which were nearly absent in normal rats .
	manualset2
82448	3	397714	5	NULL	NULL	0	NULL	OX22 - cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the nude rat CD8 + subset contained a substantial number of OX22 - cells which were nearly absent in normal rats .
	manualset2
82449	4	397714	5	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the nude rat CD8 + subset contained a substantial number of OX22 - cells which were nearly absent in normal rats .
	manualset2
82450	1	397715	5	NULL	NULL	0	NULL	pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the pain-relieved groups 2 and 4b performed statistically significantly better in PASAT than the pain-suffering groups 3 and 4a .
	manualset2
82451	2	397715	5	NULL	NULL	0	NULL	groups	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the pain-relieved groups 2 and 4b performed statistically significantly better in PASAT than the pain-suffering groups 3 and 4a .
	manualset2
82452	3	397715	5	NULL	NULL	0	NULL	PASAT	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the pain-relieved groups 2 and 4b performed statistically significantly better in PASAT than the pain-suffering groups 3 and 4a .
	manualset2
82453	4	397715	5	NULL	NULL	0	NULL	pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the pain-relieved groups 2 and 4b performed statistically significantly better in PASAT than the pain-suffering groups 3 and 4a .
	manualset2
82454	5	397715	5	NULL	NULL	0	NULL	groups	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the pain-relieved groups 2 and 4b performed statistically significantly better in PASAT than the pain-suffering groups 3 and 4a .
	manualset2
82455	1	397716	5	NULL	NULL	0	NULL	phase	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the phase coupling between multiple low-frequency signals is likely to produce a high rate of false positives when CFC is evaluated using bivariate methods .
	manualset2
82456	2	397716	5	NULL	NULL	NULL	NULL	 low-frequency signals	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the phase coupling between multiple low-frequency signals is likely to produce a high rate of false positives when CFC is evaluated using bivariate methods .
	manualset2
82457	3	397716	5	NULL	NULL	0	NULL	produce	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the phase coupling between multiple low-frequency signals is likely to produce a high rate of false positives when CFC is evaluated using bivariate methods .
	manualset2
82458	4	397716	5	NULL	NULL	NULL	NULL	CFC	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the phase coupling between multiple low-frequency signals is likely to produce a high rate of false positives when CFC is evaluated using bivariate methods .
	manualset2
82543	5	397716	5	NULL	NULL	0	NULL	bivariate methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the phase coupling between multiple low-frequency signals is likely to produce a high rate of false positives when CFC is evaluated using bivariate methods .
	manualset2
82459	1	397717	5	NULL	NULL	0	NULL	prevention	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Secondary prevention of cerebral infarct ) .
	manualset2
82460	2	397717	5	NULL	NULL	0	NULL	cerebral infarct	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Secondary prevention of cerebral infarct ) .
	manualset2
82461	1	397718	5	NULL	NULL	0	NULL	genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the presence of multiple genes for these rGH-related proteins is suggested by the large family of immunoreactive gene products identified after cell-free translation of messenger RNA derived from the pituitary .
	manualset2
82462	2	397718	5	NULL	NULL	0	NULL	rGH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the presence of multiple genes for these rGH-related proteins is suggested by the large family of immunoreactive gene products identified after cell-free translation of messenger RNA derived from the pituitary .
	manualset2
82463	3	397718	5	NULL	NULL	0	NULL	proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the presence of multiple genes for these rGH-related proteins is suggested by the large family of immunoreactive gene products identified after cell-free translation of messenger RNA derived from the pituitary .
	manualset2
82464	5	397718	5	NULL	NULL	NULL	NULL	immunoreactive gene products	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the presence of multiple genes for these rGH-related proteins is suggested by the large family of immunoreactive gene products identified after cell-free translation of messenger RNA derived from the pituitary .
	manualset2
82466	6	397718	5	NULL	NULL	0	NULL	cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the presence of multiple genes for these rGH-related proteins is suggested by the large family of immunoreactive gene products identified after cell-free translation of messenger RNA derived from the pituitary .
	manualset2
82467	7	397718	5	NULL	NULL	0	NULL	translation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the presence of multiple genes for these rGH-related proteins is suggested by the large family of immunoreactive gene products identified after cell-free translation of messenger RNA derived from the pituitary .
	manualset2
82468	8	397718	5	NULL	NULL	0	NULL	messenger RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the presence of multiple genes for these rGH-related proteins is suggested by the large family of immunoreactive gene products identified after cell-free translation of messenger RNA derived from the pituitary .
	manualset2
82469	9	397718	5	NULL	NULL	0	NULL	pituitary	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the presence of multiple genes for these rGH-related proteins is suggested by the large family of immunoreactive gene products identified after cell-free translation of messenger RNA derived from the pituitary .
	manualset2
82544	4	397718	5	NULL	NULL	0	NULL	family	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the presence of multiple genes for these rGH-related proteins is suggested by the large family of immunoreactive gene products identified after cell-free translation of messenger RNA derived from the pituitary .
	manualset2
82470	1	397719	5	NULL	NULL	0	NULL	dysplasia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the present study showed that more consensus scoring on either the degree of dysplasia , assessment of risk or the presence of each morphological characteristic by a panel should be encouraged .
	manualset2
82545	2	397719	5	NULL	NULL	0	NULL	assessment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the present study showed that more consensus scoring on either the degree of dysplasia , assessment of risk or the presence of each morphological characteristic by a panel should be encouraged .
	manualset2
82471	1	397720	5	NULL	NULL	NULL	NULL	acetyl-ACP	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the rate of acetyl-ACP-primed fatty acid synthesis was inhibited significantly by cerulenin , indicating that the slow utilization of acetyl-ACP was predominantly by 3-oxoacyl-ACP synthase I. In light-incubated isolated chloroplasts with high rates of fatty acid synthesis ( greater than 800 nmol.h-1 .
	manualset2
82472	2	397720	5	NULL	NULL	NULL	NULL	fatty acid	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the rate of acetyl-ACP-primed fatty acid synthesis was inhibited significantly by cerulenin , indicating that the slow utilization of acetyl-ACP was predominantly by 3-oxoacyl-ACP synthase I. In light-incubated isolated chloroplasts with high rates of fatty acid synthesis ( greater than 800 nmol.h-1 .
	manualset2
82473	3	397720	5	NULL	NULL	0	NULL	synthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the rate of acetyl-ACP-primed fatty acid synthesis was inhibited significantly by cerulenin , indicating that the slow utilization of acetyl-ACP was predominantly by 3-oxoacyl-ACP synthase I. In light-incubated isolated chloroplasts with high rates of fatty acid synthesis ( greater than 800 nmol.h-1 .
	manualset2
82474	4	397720	5	NULL	NULL	NULL	NULL	cerulenin	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the rate of acetyl-ACP-primed fatty acid synthesis was inhibited significantly by cerulenin , indicating that the slow utilization of acetyl-ACP was predominantly by 3-oxoacyl-ACP synthase I. In light-incubated isolated chloroplasts with high rates of fatty acid synthesis ( greater than 800 nmol.h-1 .
	manualset2
82475	5	397720	5	NULL	NULL	NULL	NULL	acetyl-ACP	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the rate of acetyl-ACP-primed fatty acid synthesis was inhibited significantly by cerulenin , indicating that the slow utilization of acetyl-ACP was predominantly by 3-oxoacyl-ACP synthase I. In light-incubated isolated chloroplasts with high rates of fatty acid synthesis ( greater than 800 nmol.h-1 .
	manualset2
82476	6	397720	5	NULL	NULL	0	NULL	3-oxoacyl-ACP synthase I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the rate of acetyl-ACP-primed fatty acid synthesis was inhibited significantly by cerulenin , indicating that the slow utilization of acetyl-ACP was predominantly by 3-oxoacyl-ACP synthase I. In light-incubated isolated chloroplasts with high rates of fatty acid synthesis ( greater than 800 nmol.h-1 .
	manualset2
82477	7	397720	5	NULL	NULL	0	NULL	light	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the rate of acetyl-ACP-primed fatty acid synthesis was inhibited significantly by cerulenin , indicating that the slow utilization of acetyl-ACP was predominantly by 3-oxoacyl-ACP synthase I. In light-incubated isolated chloroplasts with high rates of fatty acid synthesis ( greater than 800 nmol.h-1 .
	manualset2
82478	8	397720	5	NULL	NULL	0	NULL	chloroplasts	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the rate of acetyl-ACP-primed fatty acid synthesis was inhibited significantly by cerulenin , indicating that the slow utilization of acetyl-ACP was predominantly by 3-oxoacyl-ACP synthase I. In light-incubated isolated chloroplasts with high rates of fatty acid synthesis ( greater than 800 nmol.h-1 .
	manualset2
82479	9	397720	5	NULL	NULL	NULL	NULL	fatty acid	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the rate of acetyl-ACP-primed fatty acid synthesis was inhibited significantly by cerulenin , indicating that the slow utilization of acetyl-ACP was predominantly by 3-oxoacyl-ACP synthase I. In light-incubated isolated chloroplasts with high rates of fatty acid synthesis ( greater than 800 nmol.h-1 .
	manualset2
82480	10	397720	5	NULL	NULL	0	NULL	synthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the rate of acetyl-ACP-primed fatty acid synthesis was inhibited significantly by cerulenin , indicating that the slow utilization of acetyl-ACP was predominantly by 3-oxoacyl-ACP synthase I. In light-incubated isolated chloroplasts with high rates of fatty acid synthesis ( greater than 800 nmol.h-1 .
	manualset2
82481	11	397720	5	NULL	NULL	0	NULL	800 nmol.h-1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the rate of acetyl-ACP-primed fatty acid synthesis was inhibited significantly by cerulenin , indicating that the slow utilization of acetyl-ACP was predominantly by 3-oxoacyl-ACP synthase I. In light-incubated isolated chloroplasts with high rates of fatty acid synthesis ( greater than 800 nmol.h-1 .
	manualset2
82482	1	397721	5	NULL	NULL	0	NULL	dissociation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the results show that the dissociation of water on Fe ( 100 ) is a non-activated process : 0.16 eV for the zero-coverage limit and 0.03 eV when surface oxygen is present .
	manualset2
82483	2	397721	5	NULL	NULL	0	NULL	water	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the results show that the dissociation of water on Fe ( 100 ) is a non-activated process : 0.16 eV for the zero-coverage limit and 0.03 eV when surface oxygen is present .
	manualset2
82484	3	397721	5	NULL	NULL	0	NULL	Fe	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the results show that the dissociation of water on Fe ( 100 ) is a non-activated process : 0.16 eV for the zero-coverage limit and 0.03 eV when surface oxygen is present .
	manualset2
82485	5	397721	5	NULL	NULL	NULL	NULL	0.16 eV	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the results show that the dissociation of water on Fe ( 100 ) is a non-activated process : 0.16 eV for the zero-coverage limit and 0.03 eV when surface oxygen is present .
	manualset2
82486	6	397721	5	NULL	NULL	NULL	NULL	0.03 eV	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the results show that the dissociation of water on Fe ( 100 ) is a non-activated process : 0.16 eV for the zero-coverage limit and 0.03 eV when surface oxygen is present .
	manualset2
82487	7	397721	5	NULL	NULL	NULL	NULL	oxygen	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the results show that the dissociation of water on Fe ( 100 ) is a non-activated process : 0.16 eV for the zero-coverage limit and 0.03 eV when surface oxygen is present .
	manualset2
82546	4	397721	5	NULL	NULL	0	NULL	non-activated process	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the results show that the dissociation of water on Fe ( 100 ) is a non-activated process : 0.16 eV for the zero-coverage limit and 0.03 eV when surface oxygen is present .
	manualset2
82488	1	397722	5	NULL	NULL	0	NULL	spicules	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the spicules end as fairly large ovoid knobs , and vulvar flaps are present in the females .
	manualset2
82489	2	397722	5	NULL	NULL	0	NULL	ovoid knobs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the spicules end as fairly large ovoid knobs , and vulvar flaps are present in the females .
	manualset2
82490	3	397722	5	NULL	NULL	0	NULL	vulvar flaps	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the spicules end as fairly large ovoid knobs , and vulvar flaps are present in the females .
	manualset2
82491	4	397722	5	NULL	NULL	0	NULL	females	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the spicules end as fairly large ovoid knobs , and vulvar flaps are present in the females .
	manualset2
82492	1	397723	5	NULL	NULL	0	NULL	neuron	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the three neuron groups that were immunoreactive for both PV and CB , immunoreactive for PV alone and immunoreactive for CB alone were heterogeneous in their structural features such as shape and size , and no particular difference was found in their structural features among these three groups .
	manualset2
82493	2	397723	5	NULL	NULL	0	NULL	immunoreactive	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the three neuron groups that were immunoreactive for both PV and CB , immunoreactive for PV alone and immunoreactive for CB alone were heterogeneous in their structural features such as shape and size , and no particular difference was found in their structural features among these three groups .
	manualset2
82494	3	397723	5	NULL	NULL	0	NULL	PV	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the three neuron groups that were immunoreactive for both PV and CB , immunoreactive for PV alone and immunoreactive for CB alone were heterogeneous in their structural features such as shape and size , and no particular difference was found in their structural features among these three groups .
	manualset2
82495	4	397723	5	NULL	NULL	0	NULL	CB	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the three neuron groups that were immunoreactive for both PV and CB , immunoreactive for PV alone and immunoreactive for CB alone were heterogeneous in their structural features such as shape and size , and no particular difference was found in their structural features among these three groups .
	manualset2
82496	5	397723	5	NULL	NULL	0	NULL	immunoreactive	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the three neuron groups that were immunoreactive for both PV and CB , immunoreactive for PV alone and immunoreactive for CB alone were heterogeneous in their structural features such as shape and size , and no particular difference was found in their structural features among these three groups .
	manualset2
82497	6	397723	5	NULL	NULL	0	NULL	PV	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the three neuron groups that were immunoreactive for both PV and CB , immunoreactive for PV alone and immunoreactive for CB alone were heterogeneous in their structural features such as shape and size , and no particular difference was found in their structural features among these three groups .
	manualset2
82498	7	397723	5	NULL	NULL	0	NULL	immunoreactive	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the three neuron groups that were immunoreactive for both PV and CB , immunoreactive for PV alone and immunoreactive for CB alone were heterogeneous in their structural features such as shape and size , and no particular difference was found in their structural features among these three groups .
	manualset2
82499	8	397723	5	NULL	NULL	0	NULL	CB	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the three neuron groups that were immunoreactive for both PV and CB , immunoreactive for PV alone and immunoreactive for CB alone were heterogeneous in their structural features such as shape and size , and no particular difference was found in their structural features among these three groups .
	manualset2
82500	1	397724	5	NULL	NULL	NULL	NULL	pentylenetetrazol	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the threshold for pentylenetetrazol ( PTZ ) clonic convulsions was also increased in response to DPA administration .
	manualset2
82501	2	397724	5	NULL	NULL	NULL	NULL	PTZ	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the threshold for pentylenetetrazol ( PTZ ) clonic convulsions was also increased in response to DPA administration .
	manualset2
82502	3	397724	5	NULL	NULL	0	NULL	clonic convulsions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the threshold for pentylenetetrazol ( PTZ ) clonic convulsions was also increased in response to DPA administration .
	manualset2
82503	4	397724	5	NULL	NULL	0	NULL	response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the threshold for pentylenetetrazol ( PTZ ) clonic convulsions was also increased in response to DPA administration .
	manualset2
82504	5	397724	5	NULL	NULL	NULL	NULL	DPA	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the threshold for pentylenetetrazol ( PTZ ) clonic convulsions was also increased in response to DPA administration .
	manualset2
82505	6	397724	5	NULL	NULL	0	NULL	administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the threshold for pentylenetetrazol ( PTZ ) clonic convulsions was also increased in response to DPA administration .
	manualset2
82506	1	397725	5	NULL	NULL	0	NULL	dosages	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Advantages of different dosages of active metabolites in the follow-up of azathioprine treatment for Crohn disease ) .
	manualset2
82507	2	397725	5	NULL	NULL	NULL	NULL	active metabolites	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Advantages of different dosages of active metabolites in the follow-up of azathioprine treatment for Crohn disease ) .
	manualset2
82508	3	397725	5	NULL	NULL	NULL	NULL	azathioprine	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Advantages of different dosages of active metabolites in the follow-up of azathioprine treatment for Crohn disease ) .
	manualset2
82509	4	397725	5	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Advantages of different dosages of active metabolites in the follow-up of azathioprine treatment for Crohn disease ) .
	manualset2
82510	5	397725	5	NULL	NULL	0	NULL	Crohn disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Advantages of different dosages of active metabolites in the follow-up of azathioprine treatment for Crohn disease ) .
	manualset2
82511	1	397726	5	NULL	NULL	NULL	NULL	Selection	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Selection of school sites with reference to traffic noise in cities ) .
	manualset2
82512	2	397726	5	NULL	NULL	0	NULL	school	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( Selection of school sites with reference to traffic noise in cities ) .
	manualset2
82513	3	397726	5	NULL	NULL	0	NULL	traffic	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	( Selection of school sites with reference to traffic noise in cities ) .
	manualset2
82514	4	397726	5	NULL	NULL	0	NULL	noise	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	( Selection of school sites with reference to traffic noise in cities ) .
	manualset2
82515	1	397727	5	NULL	NULL	0	NULL	tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the tumor displayed evidence of close relations with the thymus capsule ; the possibility that it may arise from the thymic stroma is considered .
	manualset2
82516	2	397727	5	NULL	NULL	0	NULL	relations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the tumor displayed evidence of close relations with the thymus capsule ; the possibility that it may arise from the thymic stroma is considered .
	manualset2
82517	3	397727	5	NULL	NULL	0	NULL	thymus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the tumor displayed evidence of close relations with the thymus capsule ; the possibility that it may arise from the thymic stroma is considered .
	manualset2
82518	4	397727	5	NULL	NULL	0	NULL	capsule	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the tumor displayed evidence of close relations with the thymus capsule ; the possibility that it may arise from the thymic stroma is considered .
	manualset2
82519	5	397727	5	NULL	NULL	NULL	NULL	thymic stroma	AnatomicalPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the tumor displayed evidence of close relations with the thymus capsule ; the possibility that it may arise from the thymic stroma is considered .
	manualset2
82520	1	397728	5	NULL	NULL	0	NULL	water	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the water content was quantified using a PCA approach .
	manualset2
82521	2	397728	5	NULL	NULL	0	NULL	PCA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the water content was quantified using a PCA approach .
	manualset2
82522	1	397729	5	NULL	NULL	0	NULL	P-D MTs	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , there appeared to be a bias in the P-D MTs , with slightly more plus ends oriented distally .
	manualset2
82523	1	397730	5	NULL	NULL	NULL	NULL	magnetic mismatch negativity ( MMNm )	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , there was an increase of magnetic mismatch negativity ( MMNm ) amplitude in attended conditions and a simultaneous decrease in unattended conditions after water drinking .
	manualset2
82525	2	397730	5	NULL	NULL	NULL	NULL	water drinking	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , there was an increase of magnetic mismatch negativity ( MMNm ) amplitude in attended conditions and a simultaneous decrease in unattended conditions after water drinking .
	manualset2
82538	1	397731	5	NULL	NULL	0	NULL	nicotinic acid	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , these results indicate that nicotinic acid is a potent antidote to treat GMX1777 overdose .
	manualset2
82539	2	397731	5	NULL	NULL	NULL	NULL	potent antidote	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , these results indicate that nicotinic acid is a potent antidote to treat GMX1777 overdose .
	manualset2
82540	3	397731	5	NULL	NULL	0	NULL	treat	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , these results indicate that nicotinic acid is a potent antidote to treat GMX1777 overdose .
	manualset2
82541	4	397731	5	NULL	NULL	NULL	NULL	GMX1777 overdose	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , these results indicate that nicotinic acid is a potent antidote to treat GMX1777 overdose .
	manualset2
82560	1	397732	5	NULL	NULL	0	NULL	agonist affinity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , this is the first demonstration that agonist affinity of a GPCR and the affinity of arrestin binding to the phosphorylated receptor are regulated by distinct receptor phosphodomains .
	manualset2
82561	2	397732	5	NULL	NULL	0	NULL	GPCR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , this is the first demonstration that agonist affinity of a GPCR and the affinity of arrestin binding to the phosphorylated receptor are regulated by distinct receptor phosphodomains .
	manualset2
82562	3	397732	5	NULL	NULL	0	NULL	affinity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , this is the first demonstration that agonist affinity of a GPCR and the affinity of arrestin binding to the phosphorylated receptor are regulated by distinct receptor phosphodomains .
	manualset2
82563	4	397732	5	NULL	NULL	0	NULL	arrestin binding	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , this is the first demonstration that agonist affinity of a GPCR and the affinity of arrestin binding to the phosphorylated receptor are regulated by distinct receptor phosphodomains .
	manualset2
82564	5	397732	5	NULL	NULL	0	NULL	phosphorylated receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , this is the first demonstration that agonist affinity of a GPCR and the affinity of arrestin binding to the phosphorylated receptor are regulated by distinct receptor phosphodomains .
	manualset2
83232	6	397732	5	NULL	NULL	0	NULL	distinct receptor phosphodomains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , this is the first demonstration that agonist affinity of a GPCR and the affinity of arrestin binding to the phosphorylated receptor are regulated by distinct receptor phosphodomains .
	manualset2
82565	1	397733	5	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , this patient also had a wheeze , eosinophilia , elevation of the serum IgE level , and was positive for specific IgE to Mucor .
	manualset2
82566	2	397733	5	NULL	NULL	0	NULL	wheeze	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , this patient also had a wheeze , eosinophilia , elevation of the serum IgE level , and was positive for specific IgE to Mucor .
	manualset2
82567	3	397733	5	NULL	NULL	0	NULL	eosinophilia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , this patient also had a wheeze , eosinophilia , elevation of the serum IgE level , and was positive for specific IgE to Mucor .
	manualset2
82568	4	397733	5	NULL	NULL	0	NULL	elevation of the serum IgE level	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , this patient also had a wheeze , eosinophilia , elevation of the serum IgE level , and was positive for specific IgE to Mucor .
	manualset2
82569	5	397733	5	NULL	NULL	0	NULL	IgE	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , this patient also had a wheeze , eosinophilia , elevation of the serum IgE level , and was positive for specific IgE to Mucor .
	manualset2
82570	6	397733	5	NULL	NULL	0	NULL	Mucor	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , this patient also had a wheeze , eosinophilia , elevation of the serum IgE level , and was positive for specific IgE to Mucor .
	manualset2
82571	1	397734	5	NULL	NULL	0	NULL	rescue	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , this rescue depends on both the clathrin-binding and J domains , suggesting that the ability of Aux to bind clathrin and the Hsc70 ATPase is essential for sperm formation .
	manualset2
82572	2	397734	5	NULL	NULL	0	NULL	clathrin-binding	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , this rescue depends on both the clathrin-binding and J domains , suggesting that the ability of Aux to bind clathrin and the Hsc70 ATPase is essential for sperm formation .
	manualset2
82573	3	397734	5	NULL	NULL	0	NULL	J domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , this rescue depends on both the clathrin-binding and J domains , suggesting that the ability of Aux to bind clathrin and the Hsc70 ATPase is essential for sperm formation .
	manualset2
82574	4	397734	5	NULL	NULL	0	NULL	Aux	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , this rescue depends on both the clathrin-binding and J domains , suggesting that the ability of Aux to bind clathrin and the Hsc70 ATPase is essential for sperm formation .
	manualset2
82575	5	397734	5	NULL	NULL	0	NULL	bind	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , this rescue depends on both the clathrin-binding and J domains , suggesting that the ability of Aux to bind clathrin and the Hsc70 ATPase is essential for sperm formation .
	manualset2
82576	6	397734	5	NULL	NULL	0	NULL	clathrin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , this rescue depends on both the clathrin-binding and J domains , suggesting that the ability of Aux to bind clathrin and the Hsc70 ATPase is essential for sperm formation .
	manualset2
82577	7	397734	5	NULL	NULL	0	NULL	Hsc70 ATPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , this rescue depends on both the clathrin-binding and J domains , suggesting that the ability of Aux to bind clathrin and the Hsc70 ATPase is essential for sperm formation .
	manualset2
82578	8	397734	5	NULL	NULL	0	NULL	sperm formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , this rescue depends on both the clathrin-binding and J domains , suggesting that the ability of Aux to bind clathrin and the Hsc70 ATPase is essential for sperm formation .
	manualset2
82579	1	397735	5	NULL	NULL	0	NULL	catecholamines ( NE and EPI )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , this study also examined the possible relationships between catecholamines ( NE and EPI ) and 8-isoprostane and between IL-2 and 8-isoprostane following a combined physical and psychological challenge .
	manualset2
82580	2	397735	5	NULL	NULL	0	NULL	8-isoprostane	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , this study also examined the possible relationships between catecholamines ( NE and EPI ) and 8-isoprostane and between IL-2 and 8-isoprostane following a combined physical and psychological challenge .
	manualset2
82581	3	397735	5	NULL	NULL	0	NULL	IL-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , this study also examined the possible relationships between catecholamines ( NE and EPI ) and 8-isoprostane and between IL-2 and 8-isoprostane following a combined physical and psychological challenge .
	manualset2
82582	4	397735	5	NULL	NULL	0	NULL	8-isoprostane	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , this study also examined the possible relationships between catecholamines ( NE and EPI ) and 8-isoprostane and between IL-2 and 8-isoprostane following a combined physical and psychological challenge .
	manualset2
82583	5	397735	5	NULL	NULL	0	NULL	physical and psychological challenge	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , this study also examined the possible relationships between catecholamines ( NE and EPI ) and 8-isoprostane and between IL-2 and 8-isoprostane following a combined physical and psychological challenge .
	manualset2
82584	1	397736	5	NULL	NULL	0	NULL	titration	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , titration of this group is linked with marked spectroscopic changes unique to CIP .
	manualset2
82585	2	397736	5	NULL	NULL	0	NULL	spectroscopic changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , titration of this group is linked with marked spectroscopic changes unique to CIP .
	manualset2
82586	3	397736	5	NULL	NULL	0	NULL	CIP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , titration of this group is linked with marked spectroscopic changes unique to CIP .
	manualset2
82587	1	397737	5	NULL	NULL	0	NULL	Sensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Sensitivity to acidity of aphthous virus strains non pathogenic for swine ) .
	manualset2
82588	2	397737	5	NULL	NULL	NULL	NULL	acidity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Sensitivity to acidity of aphthous virus strains non pathogenic for swine ) .
	manualset2
82589	3	397737	5	NULL	NULL	0	NULL	aphthous virus strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Sensitivity to acidity of aphthous virus strains non pathogenic for swine ) .
	manualset2
82590	4	397737	5	NULL	NULL	0	NULL	swine	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Sensitivity to acidity of aphthous virus strains non pathogenic for swine ) .
	manualset2
82591	1	397738	5	NULL	NULL	0	NULL	anti-inflammatory action	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , to confirm the anti-inflammatory action of PPAR activated by baicalin , we used lipopolysaccharide ( LPS ) - treated cells and mice .
	manualset2
82592	2	397738	5	NULL	NULL	0	NULL	PPAR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , to confirm the anti-inflammatory action of PPAR activated by baicalin , we used lipopolysaccharide ( LPS ) - treated cells and mice .
	manualset2
82593	3	397738	5	NULL	NULL	0	NULL	baicalin	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , to confirm the anti-inflammatory action of PPAR activated by baicalin , we used lipopolysaccharide ( LPS ) - treated cells and mice .
	manualset2
82594	4	397738	5	NULL	NULL	0	NULL	lipopolysaccharide ( LPS ) - treated cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , to confirm the anti-inflammatory action of PPAR activated by baicalin , we used lipopolysaccharide ( LPS ) - treated cells and mice .
	manualset2
82595	5	397738	5	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , to confirm the anti-inflammatory action of PPAR activated by baicalin , we used lipopolysaccharide ( LPS ) - treated cells and mice .
	manualset2
82596	1	397739	5	NULL	NULL	0	NULL	treatment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , treatment with the non-promoting mitogens 4-O-methyl-TPA and Ca-ionophore A 23187 did not result in any alterations of the matrix composition .
	manualset2
82597	2	397739	5	NULL	NULL	0	NULL	non-promoting mitogens 4-O-methyl-TPA	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , treatment with the non-promoting mitogens 4-O-methyl-TPA and Ca-ionophore A 23187 did not result in any alterations of the matrix composition .
	manualset2
82598	3	397739	5	NULL	NULL	0	NULL	non-promoting mitogens Ca-ionophore A 23187	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , treatment with the non-promoting mitogens 4-O-methyl-TPA and Ca-ionophore A 23187 did not result in any alterations of the matrix composition .
	manualset2
82599	4	397739	5	NULL	NULL	0	NULL	matrix composition	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , treatment with the non-promoting mitogens 4-O-methyl-TPA and Ca-ionophore A 23187 did not result in any alterations of the matrix composition .
	manualset2
82600	1	397740	5	NULL	NULL	0	NULL	tremor power	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , tremor power accounted for a significant part of variance in the contralateral striatum , suggesting a relationship between this PD symptom and the degeneration of the dopaminergic system .
	manualset2
82601	2	397740	5	NULL	NULL	0	NULL	contralateral striatum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , tremor power accounted for a significant part of variance in the contralateral striatum , suggesting a relationship between this PD symptom and the degeneration of the dopaminergic system .
	manualset2
82602	3	397740	5	NULL	NULL	0	NULL	PD symptom	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , tremor power accounted for a significant part of variance in the contralateral striatum , suggesting a relationship between this PD symptom and the degeneration of the dopaminergic system .
	manualset2
82603	4	397740	5	NULL	NULL	0	NULL	degeneration of the dopaminergic system 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , tremor power accounted for a significant part of variance in the contralateral striatum , suggesting a relationship between this PD symptom and the degeneration of the dopaminergic system .
	manualset2
82604	1	397741	5	NULL	NULL	0	NULL	high affinity binding	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , we compare two of these double sites and show that high affinity binding of GATA-1 to a reporter gene does not necessarily induce transactivation , namely the sequence of the DNA-binding site can alter the ability of GATA-1 to stimulate transcription .
	manualset2
82605	2	397741	5	NULL	NULL	0	NULL	GATA-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , we compare two of these double sites and show that high affinity binding of GATA-1 to a reporter gene does not necessarily induce transactivation , namely the sequence of the DNA-binding site can alter the ability of GATA-1 to stimulate transcription .
	manualset2
82606	3	397741	5	NULL	NULL	0	NULL	transactivation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , we compare two of these double sites and show that high affinity binding of GATA-1 to a reporter gene does not necessarily induce transactivation , namely the sequence of the DNA-binding site can alter the ability of GATA-1 to stimulate transcription .
	manualset2
82607	4	397741	5	NULL	NULL	NULL	NULL	sequence of the DNA-binding site	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , we compare two of these double sites and show that high affinity binding of GATA-1 to a reporter gene does not necessarily induce transactivation , namely the sequence of the DNA-binding site can alter the ability of GATA-1 to stimulate transcription .
	manualset2
82608	5	397741	5	NULL	NULL	0	NULL	GATA-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , we compare two of these double sites and show that high affinity binding of GATA-1 to a reporter gene does not necessarily induce transactivation , namely the sequence of the DNA-binding site can alter the ability of GATA-1 to stimulate transcription .
	manualset2
82609	6	397741	5	NULL	NULL	0	NULL	transcription	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , we compare two of these double sites and show that high affinity binding of GATA-1 to a reporter gene does not necessarily induce transactivation , namely the sequence of the DNA-binding site can alter the ability of GATA-1 to stimulate transcription .
	manualset2
82610	1	397742	5	NULL	NULL	0	NULL	alk1 expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , we demonstrate that alk1 expression requires blood flow , and despite normal levels of shear stress , some flow-responsive genes are dysregulated in alk1 mutant arterial endothelial cells .
	manualset2
82611	3	397742	5	NULL	NULL	NULL	NULL	shear stress	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , we demonstrate that alk1 expression requires blood flow , and despite normal levels of shear stress , some flow-responsive genes are dysregulated in alk1 mutant arterial endothelial cells .
	manualset2
82612	4	397742	5	NULL	NULL	NULL	NULL	flow-responsive genes	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , we demonstrate that alk1 expression requires blood flow , and despite normal levels of shear stress , some flow-responsive genes are dysregulated in alk1 mutant arterial endothelial cells .
	manualset2
82613	5	397742	5	NULL	NULL	NULL	NULL	alk1 mutant arterial endothelial cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , we demonstrate that alk1 expression requires blood flow , and despite normal levels of shear stress , some flow-responsive genes are dysregulated in alk1 mutant arterial endothelial cells .
	manualset2
82614	2	397742	5	NULL	NULL	0	NULL	blood flow	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , we demonstrate that alk1 expression requires blood flow , and despite normal levels of shear stress , some flow-responsive genes are dysregulated in alk1 mutant arterial endothelial cells .
	manualset2
82615	1	397743	5	NULL	NULL	0	NULL	Bcl-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , we have targeted Bcl-2 specifically to either the ER or the outer mitochondrial membrane to test whether induction of apoptosis by Bcl-2 is dependent upon its localization within either of these membranes .
	manualset2
82616	2	397743	5	NULL	NULL	0	NULL	ER	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , we have targeted Bcl-2 specifically to either the ER or the outer mitochondrial membrane to test whether induction of apoptosis by Bcl-2 is dependent upon its localization within either of these membranes .
	manualset2
82617	3	397743	5	NULL	NULL	0	NULL	outer mitochondrial membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , we have targeted Bcl-2 specifically to either the ER or the outer mitochondrial membrane to test whether induction of apoptosis by Bcl-2 is dependent upon its localization within either of these membranes .
	manualset2
82618	4	397743	5	NULL	NULL	0	NULL	induction of apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , we have targeted Bcl-2 specifically to either the ER or the outer mitochondrial membrane to test whether induction of apoptosis by Bcl-2 is dependent upon its localization within either of these membranes .
	manualset2
82619	5	397743	5	NULL	NULL	0	NULL	Bcl-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , we have targeted Bcl-2 specifically to either the ER or the outer mitochondrial membrane to test whether induction of apoptosis by Bcl-2 is dependent upon its localization within either of these membranes .
	manualset2
82620	6	397743	5	NULL	NULL	0	NULL	localization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , we have targeted Bcl-2 specifically to either the ER or the outer mitochondrial membrane to test whether induction of apoptosis by Bcl-2 is dependent upon its localization within either of these membranes .
	manualset2
82621	7	397743	5	NULL	NULL	0	NULL	membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , we have targeted Bcl-2 specifically to either the ER or the outer mitochondrial membrane to test whether induction of apoptosis by Bcl-2 is dependent upon its localization within either of these membranes .
	manualset2
82622	1	397744	5	NULL	NULL	0	NULL	isolate	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , we planned to isolate and identify the neuroprotective agent from LBP using chromatographic methods .
	manualset2
82623	2	397744	5	NULL	NULL	0	NULL	identify	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , we planned to isolate and identify the neuroprotective agent from LBP using chromatographic methods .
	manualset2
82624	3	397744	5	NULL	NULL	0	NULL	neuroprotective agent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , we planned to isolate and identify the neuroprotective agent from LBP using chromatographic methods .
	manualset2
82625	4	397744	5	NULL	NULL	0	NULL	LBP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , we planned to isolate and identify the neuroprotective agent from LBP using chromatographic methods .
	manualset2
82626	5	397744	5	NULL	NULL	0	NULL	chromatographic methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , we planned to isolate and identify the neuroprotective agent from LBP using chromatographic methods .
	manualset2
82628	1	397745	5	NULL	NULL	NULL	NULL	STU	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , we present evidence that STU serves as an important regulator mediating the control of cell proliferation by GA possibly through two cyclin-dependent kinase inhibitors , SIM and SMR1 .
	manualset2
82630	2	397745	5	NULL	NULL	NULL	NULL	important regulator	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , we present evidence that STU serves as an important regulator mediating the control of cell proliferation by GA possibly through two cyclin-dependent kinase inhibitors , SIM and SMR1 .
	manualset2
82631	3	397745	5	NULL	NULL	NULL	NULL	control of cell proliferation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , we present evidence that STU serves as an important regulator mediating the control of cell proliferation by GA possibly through two cyclin-dependent kinase inhibitors , SIM and SMR1 .
	manualset2
82633	4	397745	5	NULL	NULL	NULL	NULL	GA	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , we present evidence that STU serves as an important regulator mediating the control of cell proliferation by GA possibly through two cyclin-dependent kinase inhibitors , SIM and SMR1 .
	manualset2
82634	5	397745	5	NULL	NULL	NULL	NULL	cyclin-dependent kinase inhibitors	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , we present evidence that STU serves as an important regulator mediating the control of cell proliferation by GA possibly through two cyclin-dependent kinase inhibitors , SIM and SMR1 .
	manualset2
82635	6	397745	5	NULL	NULL	NULL	NULL	SIM	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , we present evidence that STU serves as an important regulator mediating the control of cell proliferation by GA possibly through two cyclin-dependent kinase inhibitors , SIM and SMR1 .
	manualset2
82636	7	397745	5	NULL	NULL	NULL	NULL	SMR1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , we present evidence that STU serves as an important regulator mediating the control of cell proliferation by GA possibly through two cyclin-dependent kinase inhibitors , SIM and SMR1 .
	manualset2
82637	1	397746	5	NULL	NULL	NULL	NULL	CsgG	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , we show that CsgG belongs to the nascent class of helical outer-membrane macromolecular exporters .
	manualset2
82639	2	397746	5	NULL	NULL	NULL	NULL	helical outer-membrane macromolecular exporters	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , we show that CsgG belongs to the nascent class of helical outer-membrane macromolecular exporters .
	manualset2
82640	1	397747	5	NULL	NULL	0	NULL	Serological types of strains of B. pertussis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Serological types of strains of B. pertussis isolated in the Warsaw area and evaluation of their histamine-sensitisation potential for mice ) .
	manualset2
82641	2	397747	5	NULL	NULL	0	NULL	Warsaw area	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Serological types of strains of B. pertussis isolated in the Warsaw area and evaluation of their histamine-sensitisation potential for mice ) .
	manualset2
82642	3	397747	5	NULL	NULL	0	NULL	evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Serological types of strains of B. pertussis isolated in the Warsaw area and evaluation of their histamine-sensitisation potential for mice ) .
	manualset2
82643	4	397747	5	NULL	NULL	0	NULL	histamine-sensitisation potential	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Serological types of strains of B. pertussis isolated in the Warsaw area and evaluation of their histamine-sensitisation potential for mice ) .
	manualset2
82644	5	397747	5	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Serological types of strains of B. pertussis isolated in the Warsaw area and evaluation of their histamine-sensitisation potential for mice ) .
	manualset2
82645	1	397748	5	NULL	NULL	0	NULL	c-Jun	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , we show that a mutated form of c-Jun lacking the transactivation domain ( TAM-67 ) was a much stronger activator of the IL-6 promoter than c-Jun .
	manualset2
82646	2	397748	5	NULL	NULL	0	NULL	transactivation domain ( TAM-67 )	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , we show that a mutated form of c-Jun lacking the transactivation domain ( TAM-67 ) was a much stronger activator of the IL-6 promoter than c-Jun .
	manualset2
82647	3	397748	5	NULL	NULL	0	NULL	stronger activator	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , we show that a mutated form of c-Jun lacking the transactivation domain ( TAM-67 ) was a much stronger activator of the IL-6 promoter than c-Jun .
	manualset2
82648	4	397748	5	NULL	NULL	0	NULL	IL-6 promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , we show that a mutated form of c-Jun lacking the transactivation domain ( TAM-67 ) was a much stronger activator of the IL-6 promoter than c-Jun .
	manualset2
82649	5	397748	5	NULL	NULL	0	NULL	c-Jun	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , we show that a mutated form of c-Jun lacking the transactivation domain ( TAM-67 ) was a much stronger activator of the IL-6 promoter than c-Jun .
	manualset2
82650	1	397749	5	NULL	NULL	0	NULL	RASSF2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , we showed that RASSF2 and MST2 do indeed colocalize , but whereas RASSF2 alone is nuclear , the presence of MST1 or MST2 results in colocalization in the cytoplasm .
	manualset2
82651	2	397749	5	NULL	NULL	0	NULL	MST2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , we showed that RASSF2 and MST2 do indeed colocalize , but whereas RASSF2 alone is nuclear , the presence of MST1 or MST2 results in colocalization in the cytoplasm .
	manualset2
82653	3	397749	5	NULL	NULL	NULL	NULL	RASSF2	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , we showed that RASSF2 and MST2 do indeed colocalize , but whereas RASSF2 alone is nuclear , the presence of MST1 or MST2 results in colocalization in the cytoplasm .
	manualset2
82654	4	397749	5	NULL	NULL	NULL	NULL	MST1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , we showed that RASSF2 and MST2 do indeed colocalize , but whereas RASSF2 alone is nuclear , the presence of MST1 or MST2 results in colocalization in the cytoplasm .
	manualset2
82655	5	397749	5	NULL	NULL	NULL	NULL	MST2	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , we showed that RASSF2 and MST2 do indeed colocalize , but whereas RASSF2 alone is nuclear , the presence of MST1 or MST2 results in colocalization in the cytoplasm .
	manualset2
82656	6	397749	5	NULL	NULL	NULL	NULL	colocalization	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , we showed that RASSF2 and MST2 do indeed colocalize , but whereas RASSF2 alone is nuclear , the presence of MST1 or MST2 results in colocalization in the cytoplasm .
	manualset2
82657	7	397749	5	NULL	NULL	NULL	NULL	cytoplasm	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , we showed that RASSF2 and MST2 do indeed colocalize , but whereas RASSF2 alone is nuclear , the presence of MST1 or MST2 results in colocalization in the cytoplasm .
	manualset2
82658	1	397750	5	NULL	NULL	0	NULL	 western blotting	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , western blotting was performed to evaluate the expression of NFB and COX-2 in testes .
	manualset2
82660	2	397750	5	NULL	NULL	NULL	NULL	expression	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , western blotting was performed to evaluate the expression of NFB and COX-2 in testes .
	manualset2
82661	3	397750	5	NULL	NULL	NULL	NULL	NFB	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , western blotting was performed to evaluate the expression of NFB and COX-2 in testes .
	manualset2
82662	4	397750	5	NULL	NULL	NULL	NULL	COX-2	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , western blotting was performed to evaluate the expression of NFB and COX-2 in testes .
	manualset2
82663	5	397750	5	NULL	NULL	NULL	NULL	testes	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , western blotting was performed to evaluate the expression of NFB and COX-2 in testes .
	manualset2
82664	1	397751	5	NULL	NULL	0	NULL	endocytosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , when endocytosis and lysosomal destabilization were inhibited , inflammasome activity was diminished , supporting the notion that nanoparticles rupture lysosomal compartments and behave as ` danger signals ' ( Hornung V , Bauernfeind F , Halle A , Samstad EO , Kono H , Rock KL , et al. .
	manualset2
82665	2	397751	5	NULL	NULL	0	NULL	lysosomal destabilization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , when endocytosis and lysosomal destabilization were inhibited , inflammasome activity was diminished , supporting the notion that nanoparticles rupture lysosomal compartments and behave as ` danger signals ' ( Hornung V , Bauernfeind F , Halle A , Samstad EO , Kono H , Rock KL , et al. .
	manualset2
82666	3	397751	5	NULL	NULL	0	NULL	inflammasome activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , when endocytosis and lysosomal destabilization were inhibited , inflammasome activity was diminished , supporting the notion that nanoparticles rupture lysosomal compartments and behave as ` danger signals ' ( Hornung V , Bauernfeind F , Halle A , Samstad EO , Kono H , Rock KL , et al. .
	manualset2
82669	4	397751	5	NULL	NULL	NULL	NULL	lysosomal compartments	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , when endocytosis and lysosomal destabilization were inhibited , inflammasome activity was diminished , supporting the notion that nanoparticles rupture lysosomal compartments and behave as ` danger signals ' ( Hornung V , Bauernfeind F , Halle A , Samstad EO , Kono H , Rock KL , et al. .
	manualset2
82670	5	397751	5	NULL	NULL	NULL	NULL	danger signals	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , when endocytosis and lysosomal destabilization were inhibited , inflammasome activity was diminished , supporting the notion that nanoparticles rupture lysosomal compartments and behave as ` danger signals ' ( Hornung V , Bauernfeind F , Halle A , Samstad EO , Kono H , Rock KL , et al. .
	manualset2
82671	1	397752	5	NULL	NULL	0	NULL	accumulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , while the accumulation of CD8 + T cells in the neural parenchyma was significantly delayed in both CXCR3 - and CXCR3/CCR5-deficient mice , more CD8 + T cells were found in the parenchyma of double-deficient mice when these were analyzed around the time when the difference in clinical outcome becomes manifest .
	manualset2
82672	2	397752	5	NULL	NULL	0	NULL	CD8 + T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , while the accumulation of CD8 + T cells in the neural parenchyma was significantly delayed in both CXCR3 - and CXCR3/CCR5-deficient mice , more CD8 + T cells were found in the parenchyma of double-deficient mice when these were analyzed around the time when the difference in clinical outcome becomes manifest .
	manualset2
82673	3	397752	5	NULL	NULL	0	NULL	neural parenchyma	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , while the accumulation of CD8 + T cells in the neural parenchyma was significantly delayed in both CXCR3 - and CXCR3/CCR5-deficient mice , more CD8 + T cells were found in the parenchyma of double-deficient mice when these were analyzed around the time when the difference in clinical outcome becomes manifest .
	manualset2
82674	4	397752	5	NULL	NULL	NULL	NULL	CXCR3 - and CXCR3/CCR5-deficient mice	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , while the accumulation of CD8 + T cells in the neural parenchyma was significantly delayed in both CXCR3 - and CXCR3/CCR5-deficient mice , more CD8 + T cells were found in the parenchyma of double-deficient mice when these were analyzed around the time when the difference in clinical outcome becomes manifest .
	manualset2
82675	5	397752	5	NULL	NULL	0	NULL	CD8 + T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , while the accumulation of CD8 + T cells in the neural parenchyma was significantly delayed in both CXCR3 - and CXCR3/CCR5-deficient mice , more CD8 + T cells were found in the parenchyma of double-deficient mice when these were analyzed around the time when the difference in clinical outcome becomes manifest .
	manualset2
82676	6	397752	5	NULL	NULL	0	NULL	parenchyma	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , while the accumulation of CD8 + T cells in the neural parenchyma was significantly delayed in both CXCR3 - and CXCR3/CCR5-deficient mice , more CD8 + T cells were found in the parenchyma of double-deficient mice when these were analyzed around the time when the difference in clinical outcome becomes manifest .
	manualset2
82677	7	397752	5	NULL	NULL	0	NULL	double-deficient mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , while the accumulation of CD8 + T cells in the neural parenchyma was significantly delayed in both CXCR3 - and CXCR3/CCR5-deficient mice , more CD8 + T cells were found in the parenchyma of double-deficient mice when these were analyzed around the time when the difference in clinical outcome becomes manifest .
	manualset2
82678	8	397752	5	NULL	NULL	NULL	NULL	around the time	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , while the accumulation of CD8 + T cells in the neural parenchyma was significantly delayed in both CXCR3 - and CXCR3/CCR5-deficient mice , more CD8 + T cells were found in the parenchyma of double-deficient mice when these were analyzed around the time when the difference in clinical outcome becomes manifest .
	manualset2
82679	9	397752	5	NULL	NULL	0	NULL	clinical outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , while the accumulation of CD8 + T cells in the neural parenchyma was significantly delayed in both CXCR3 - and CXCR3/CCR5-deficient mice , more CD8 + T cells were found in the parenchyma of double-deficient mice when these were analyzed around the time when the difference in clinical outcome becomes manifest .
	manualset2
82743	1	397753	5	NULL	NULL	0	NULL	Ang II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore Ang II and CGP 42112 have no effect on nitroprusside-stimulated cGMP levels in these cells , thus ruling out interactions between the AT2 receptor and soluble guanylate cyclase .
	manualset2
82744	2	397753	5	NULL	NULL	0	NULL	CGP 42112	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore Ang II and CGP 42112 have no effect on nitroprusside-stimulated cGMP levels in these cells , thus ruling out interactions between the AT2 receptor and soluble guanylate cyclase .
	manualset2
82745	3	397753	5	NULL	NULL	NULL	NULL	nitroprusside-stimulated cGMP levels	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore Ang II and CGP 42112 have no effect on nitroprusside-stimulated cGMP levels in these cells , thus ruling out interactions between the AT2 receptor and soluble guanylate cyclase .
	manualset2
82746	4	397753	5	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore Ang II and CGP 42112 have no effect on nitroprusside-stimulated cGMP levels in these cells , thus ruling out interactions between the AT2 receptor and soluble guanylate cyclase .
	manualset2
82747	5	397753	5	NULL	NULL	0	NULL	interactions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore Ang II and CGP 42112 have no effect on nitroprusside-stimulated cGMP levels in these cells , thus ruling out interactions between the AT2 receptor and soluble guanylate cyclase .
	manualset2
82748	6	397753	5	NULL	NULL	0	NULL	AT2 receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore Ang II and CGP 42112 have no effect on nitroprusside-stimulated cGMP levels in these cells , thus ruling out interactions between the AT2 receptor and soluble guanylate cyclase .
	manualset2
82749	7	397753	5	NULL	NULL	0	NULL	soluble guanylate cyclase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore Ang II and CGP 42112 have no effect on nitroprusside-stimulated cGMP levels in these cells , thus ruling out interactions between the AT2 receptor and soluble guanylate cyclase .
	manualset2
82750	1	397754	5	NULL	NULL	0	NULL	cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore cell lines derived from IL-7 transgenic mice may provide a novel source of rare factor-dependent bipotent stem cells .
	manualset2
82751	2	397754	5	NULL	NULL	0	NULL	IL-7 transgenic mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore cell lines derived from IL-7 transgenic mice may provide a novel source of rare factor-dependent bipotent stem cells .
	manualset2
82752	3	397754	5	NULL	NULL	0	NULL	factor-dependent bipotent stem cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore cell lines derived from IL-7 transgenic mice may provide a novel source of rare factor-dependent bipotent stem cells .
	manualset2
82753	1	397755	5	NULL	NULL	0	NULL	hypoalbuminemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore hypoalbuminemia due to severe anorexia might have enhanced the occurrence of the disease .
	manualset2
82754	2	397755	5	NULL	NULL	0	NULL	severe anorexia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore hypoalbuminemia due to severe anorexia might have enhanced the occurrence of the disease .
	manualset2
82755	3	397755	5	NULL	NULL	0	NULL	occurrence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore hypoalbuminemia due to severe anorexia might have enhanced the occurrence of the disease .
	manualset2
82756	4	397755	5	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore hypoalbuminemia due to severe anorexia might have enhanced the occurrence of the disease .
	manualset2
82757	1	397756	5	NULL	NULL	0	NULL	Serum hormonal activities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Serum hormonal activities in normal women and in patients with breast cancer ) .
	manualset2
82758	2	397756	5	NULL	NULL	0	NULL	normal women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Serum hormonal activities in normal women and in patients with breast cancer ) .
	manualset2
82759	3	397756	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Serum hormonal activities in normal women and in patients with breast cancer ) .
	manualset2
82760	4	397756	5	NULL	NULL	0	NULL	breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Serum hormonal activities in normal women and in patients with breast cancer ) .
	manualset2
82761	1	397757	5	NULL	NULL	0	NULL	 palisade ending-MIF unit	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore the ` palisade ending-MIF unit ' may be part of a sensory feedback system in eye muscles , which should be considered in association with the causes and treatment of strabismus .
	manualset2
82762	2	397757	5	NULL	NULL	0	NULL	sensory feedback system	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore the ` palisade ending-MIF unit ' may be part of a sensory feedback system in eye muscles , which should be considered in association with the causes and treatment of strabismus .
	manualset2
82763	3	397757	5	NULL	NULL	0	NULL	eye muscles	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore the ` palisade ending-MIF unit ' may be part of a sensory feedback system in eye muscles , which should be considered in association with the causes and treatment of strabismus .
	manualset2
82764	4	397757	5	NULL	NULL	0	NULL	causes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore the ` palisade ending-MIF unit ' may be part of a sensory feedback system in eye muscles , which should be considered in association with the causes and treatment of strabismus .
	manualset2
82765	5	397757	5	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore the ` palisade ending-MIF unit ' may be part of a sensory feedback system in eye muscles , which should be considered in association with the causes and treatment of strabismus .
	manualset2
82766	6	397757	5	NULL	NULL	0	NULL	strabismus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore the ` palisade ending-MIF unit ' may be part of a sensory feedback system in eye muscles , which should be considered in association with the causes and treatment of strabismus .
	manualset2
82767	1	397758	5	NULL	NULL	0	NULL	Fusarium oxysporum homogenates	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Fusarium oxysporum homogenates and jasmonate induce limited sanguinarine accumulation in Argemone mexicana cell cultures .
	manualset2
82768	2	397758	5	NULL	NULL	0	NULL	jasmonate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Fusarium oxysporum homogenates and jasmonate induce limited sanguinarine accumulation in Argemone mexicana cell cultures .
	manualset2
82769	3	397758	5	NULL	NULL	0	NULL	sanguinarine accumulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fusarium oxysporum homogenates and jasmonate induce limited sanguinarine accumulation in Argemone mexicana cell cultures .
	manualset2
82770	4	397758	5	NULL	NULL	0	NULL	Argemone mexicana cell cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Fusarium oxysporum homogenates and jasmonate induce limited sanguinarine accumulation in Argemone mexicana cell cultures .
	manualset2
82771	1	397759	5	NULL	NULL	0	NULL	Fusion	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Fusion of secretion signals to the reporter cloned in a shuttle vector , pBPnuc1 , resulted in halo formation around colonies of Mycobacterium smegmatis and Mycobacterium tuberculosis grown on DNase agar plates containing Methyl Green indicator dye .
	manualset2
82772	2	397759	5	NULL	NULL	0	NULL	secretion signals	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fusion of secretion signals to the reporter cloned in a shuttle vector , pBPnuc1 , resulted in halo formation around colonies of Mycobacterium smegmatis and Mycobacterium tuberculosis grown on DNase agar plates containing Methyl Green indicator dye .
	manualset2
82773	3	397759	5	NULL	NULL	0	NULL	reporter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Fusion of secretion signals to the reporter cloned in a shuttle vector , pBPnuc1 , resulted in halo formation around colonies of Mycobacterium smegmatis and Mycobacterium tuberculosis grown on DNase agar plates containing Methyl Green indicator dye .
	manualset2
82774	4	397759	5	NULL	NULL	NULL	NULL	shuttle vector , pBPnuc1 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fusion of secretion signals to the reporter cloned in a shuttle vector , pBPnuc1 , resulted in halo formation around colonies of Mycobacterium smegmatis and Mycobacterium tuberculosis grown on DNase agar plates containing Methyl Green indicator dye .
	manualset2
82775	5	397759	5	NULL	NULL	0	NULL	halo formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fusion of secretion signals to the reporter cloned in a shuttle vector , pBPnuc1 , resulted in halo formation around colonies of Mycobacterium smegmatis and Mycobacterium tuberculosis grown on DNase agar plates containing Methyl Green indicator dye .
	manualset2
82776	6	397759	5	NULL	NULL	0	NULL	colonies of Mycobacterium smegmatis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Fusion of secretion signals to the reporter cloned in a shuttle vector , pBPnuc1 , resulted in halo formation around colonies of Mycobacterium smegmatis and Mycobacterium tuberculosis grown on DNase agar plates containing Methyl Green indicator dye .
	manualset2
82777	7	397759	5	NULL	NULL	0	NULL	Mycobacterium tuberculosis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Fusion of secretion signals to the reporter cloned in a shuttle vector , pBPnuc1 , resulted in halo formation around colonies of Mycobacterium smegmatis and Mycobacterium tuberculosis grown on DNase agar plates containing Methyl Green indicator dye .
	manualset2
82778	8	397759	5	NULL	NULL	0	NULL	DNase agar plates	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Fusion of secretion signals to the reporter cloned in a shuttle vector , pBPnuc1 , resulted in halo formation around colonies of Mycobacterium smegmatis and Mycobacterium tuberculosis grown on DNase agar plates containing Methyl Green indicator dye .
	manualset2
82779	9	397759	5	NULL	NULL	0	NULL	Methyl Green indicator dye	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Fusion of secretion signals to the reporter cloned in a shuttle vector , pBPnuc1 , resulted in halo formation around colonies of Mycobacterium smegmatis and Mycobacterium tuberculosis grown on DNase agar plates containing Methyl Green indicator dye .
	manualset2
82781	1	397760	5	NULL	NULL	NULL	NULL	designing models of care and infrastructure	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Future policy directions include designing models of care and infrastructure that enable patients and their family carers to balance life and illness , and aligning patient-centred care not only within health services but also with community and social support services .
	manualset2
82783	2	397760	5	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Future policy directions include designing models of care and infrastructure that enable patients and their family carers to balance life and illness , and aligning patient-centred care not only within health services but also with community and social support services .
	manualset2
82784	3	397760	5	NULL	NULL	NULL	NULL	family carers	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Future policy directions include designing models of care and infrastructure that enable patients and their family carers to balance life and illness , and aligning patient-centred care not only within health services but also with community and social support services .
	manualset2
82786	4	397760	5	NULL	NULL	NULL	NULL	life	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Future policy directions include designing models of care and infrastructure that enable patients and their family carers to balance life and illness , and aligning patient-centred care not only within health services but also with community and social support services .
	manualset2
82787	5	397760	5	NULL	NULL	NULL	NULL	illness	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Future policy directions include designing models of care and infrastructure that enable patients and their family carers to balance life and illness , and aligning patient-centred care not only within health services but also with community and social support services .
	manualset2
82788	6	397760	5	NULL	NULL	NULL	NULL	patient-centred care	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Future policy directions include designing models of care and infrastructure that enable patients and their family carers to balance life and illness , and aligning patient-centred care not only within health services but also with community and social support services .
	manualset2
82789	7	397760	5	NULL	NULL	NULL	NULL	health services	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Future policy directions include designing models of care and infrastructure that enable patients and their family carers to balance life and illness , and aligning patient-centred care not only within health services but also with community and social support services .
	manualset2
82790	8	397760	5	NULL	NULL	NULL	NULL	community	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Future policy directions include designing models of care and infrastructure that enable patients and their family carers to balance life and illness , and aligning patient-centred care not only within health services but also with community and social support services .
	manualset2
82791	9	397760	5	NULL	NULL	NULL	NULL	social support services	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Future policy directions include designing models of care and infrastructure that enable patients and their family carers to balance life and illness , and aligning patient-centred care not only within health services but also with community and social support services .
	manualset2
82792	1	397761	5	NULL	NULL	0	NULL	Future research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Future research should be aimed at developing vaccines that approach the ideal as closely as possible and which are directed against diseases not yet controlled by vaccination and against newly emerging diseases .
	manualset2
82794	3	397761	5	NULL	NULL	0	NULL	diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Future research should be aimed at developing vaccines that approach the ideal as closely as possible and which are directed against diseases not yet controlled by vaccination and against newly emerging diseases .
	manualset2
82795	4	397761	5	NULL	NULL	0	NULL	vaccination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Future research should be aimed at developing vaccines that approach the ideal as closely as possible and which are directed against diseases not yet controlled by vaccination and against newly emerging diseases .
	manualset2
82796	5	397761	5	NULL	NULL	0	NULL	newly emerging diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Future research should be aimed at developing vaccines that approach the ideal as closely as possible and which are directed against diseases not yet controlled by vaccination and against newly emerging diseases .
	manualset2
83114	2	397761	5	NULL	NULL	0	NULL	vaccines	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Future research should be aimed at developing vaccines that approach the ideal as closely as possible and which are directed against diseases not yet controlled by vaccination and against newly emerging diseases .
	manualset2
82797	1	397762	5	NULL	NULL	NULL	NULL	Future studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Future studies should assess primarily the efficacy and safety of aspirin in essential thrombocythemia , and test the possible use of more aggressive antithrombotic strategies in high-risk polycythemic patients .
	manualset2
82798	2	397762	5	NULL	NULL	NULL	NULL	efficacy and safety	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Future studies should assess primarily the efficacy and safety of aspirin in essential thrombocythemia , and test the possible use of more aggressive antithrombotic strategies in high-risk polycythemic patients .
	manualset2
82800	3	397762	5	NULL	NULL	NULL	NULL	aspirin	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Future studies should assess primarily the efficacy and safety of aspirin in essential thrombocythemia , and test the possible use of more aggressive antithrombotic strategies in high-risk polycythemic patients .
	manualset2
82801	4	397762	5	NULL	NULL	NULL	NULL	essential thrombocythemia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Future studies should assess primarily the efficacy and safety of aspirin in essential thrombocythemia , and test the possible use of more aggressive antithrombotic strategies in high-risk polycythemic patients .
	manualset2
82802	5	397762	5	NULL	NULL	NULL	NULL	test	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Future studies should assess primarily the efficacy and safety of aspirin in essential thrombocythemia , and test the possible use of more aggressive antithrombotic strategies in high-risk polycythemic patients .
	manualset2
82803	6	397762	5	NULL	NULL	NULL	NULL	more aggressive antithrombotic strategies	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Future studies should assess primarily the efficacy and safety of aspirin in essential thrombocythemia , and test the possible use of more aggressive antithrombotic strategies in high-risk polycythemic patients .
	manualset2
82804	7	397762	5	NULL	NULL	NULL	NULL	high-risk polycythemic patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Future studies should assess primarily the efficacy and safety of aspirin in essential thrombocythemia , and test the possible use of more aggressive antithrombotic strategies in high-risk polycythemic patients .
	manualset2
82805	1	397763	5	NULL	NULL	0	NULL	complex relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Future studies should shed new light on the complex relationship between HPTMs and human development .
	manualset2
82806	2	397763	5	NULL	NULL	0	NULL	HPTMs	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Future studies should shed new light on the complex relationship between HPTMs and human development .
	manualset2
82807	3	397763	5	NULL	NULL	0	NULL	human	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Future studies should shed new light on the complex relationship between HPTMs and human development .
	manualset2
82808	4	397763	5	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Future studies should shed new light on the complex relationship between HPTMs and human development .
	manualset2
82809	1	397764	5	NULL	NULL	0	NULL	theoretical developments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Future theoretical developments that move away from an abstract foundation embedded in cost-benefit tradeoffs and toward phenotypic integration of source-sink relationships will improve our ability to merge observations and theory .
	manualset2
82810	2	397764	5	NULL	NULL	0	NULL	abstract foundation	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Future theoretical developments that move away from an abstract foundation embedded in cost-benefit tradeoffs and toward phenotypic integration of source-sink relationships will improve our ability to merge observations and theory .
	manualset2
82811	3	397764	5	NULL	NULL	0	NULL	cost-benefit tradeoffs	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Future theoretical developments that move away from an abstract foundation embedded in cost-benefit tradeoffs and toward phenotypic integration of source-sink relationships will improve our ability to merge observations and theory .
	manualset2
82812	4	397764	5	NULL	NULL	0	NULL	phenotypic integration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Future theoretical developments that move away from an abstract foundation embedded in cost-benefit tradeoffs and toward phenotypic integration of source-sink relationships will improve our ability to merge observations and theory .
	manualset2
82813	5	397764	5	NULL	NULL	0	NULL	source-sink relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Future theoretical developments that move away from an abstract foundation embedded in cost-benefit tradeoffs and toward phenotypic integration of source-sink relationships will improve our ability to merge observations and theory .
	manualset2
82814	6	397764	5	NULL	NULL	0	NULL	observations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Future theoretical developments that move away from an abstract foundation embedded in cost-benefit tradeoffs and toward phenotypic integration of source-sink relationships will improve our ability to merge observations and theory .
	manualset2
82815	7	397764	5	NULL	NULL	0	NULL	theory	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Future theoretical developments that move away from an abstract foundation embedded in cost-benefit tradeoffs and toward phenotypic integration of source-sink relationships will improve our ability to merge observations and theory .
	manualset2
82816	1	397765	5	NULL	NULL	0	NULL	Serum level	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	( Serum level of alpha-1 antitrypsin in patients with sarcoidosis ) .
	manualset2
82817	2	397765	5	NULL	NULL	0	NULL	alpha-1 antitrypsin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Serum level of alpha-1 antitrypsin in patients with sarcoidosis ) .
	manualset2
82818	3	397765	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Serum level of alpha-1 antitrypsin in patients with sarcoidosis ) .
	manualset2
82819	4	397765	5	NULL	NULL	0	NULL	sarcoidosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Serum level of alpha-1 antitrypsin in patients with sarcoidosis ) .
	manualset2
82820	1	397766	5	NULL	NULL	0	NULL	local bone regeneration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Future of local bone regeneration - Protein versus gene therapy .
	manualset2
82821	2	397766	5	NULL	NULL	0	NULL	Protein therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Future of local bone regeneration - Protein versus gene therapy .
	manualset2
82822	3	397766	5	NULL	NULL	0	NULL	gene therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Future of local bone regeneration - Protein versus gene therapy .
	manualset2
82823	1	397767	5	NULL	NULL	0	NULL	GA	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	GA has been shown to reduce alpha-synuclein induced neurotoxicity in a fly model of Parkinson 's disease .
	manualset2
82824	2	397767	5	NULL	NULL	0	NULL	alpha-synuclein induced neurotoxicity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GA has been shown to reduce alpha-synuclein induced neurotoxicity in a fly model of Parkinson 's disease .
	manualset2
82825	3	397767	5	NULL	NULL	0	NULL	fly model	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	GA has been shown to reduce alpha-synuclein induced neurotoxicity in a fly model of Parkinson 's disease .
	manualset2
82826	4	397767	5	NULL	NULL	0	NULL	Parkinson 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	GA has been shown to reduce alpha-synuclein induced neurotoxicity in a fly model of Parkinson 's disease .
	manualset2
82827	1	397768	5	NULL	NULL	0	NULL	GABA	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	GABA hyperpolarizes hippocampal CA1 and CA3 pyramidal cells through activation of GABAB postsynaptic receptors .
	manualset2
82828	2	397768	5	NULL	NULL	0	NULL	 hippocampal CA1 and CA3 pyramidal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	GABA hyperpolarizes hippocampal CA1 and CA3 pyramidal cells through activation of GABAB postsynaptic receptors .
	manualset2
82829	3	397768	5	NULL	NULL	0	NULL	activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GABA hyperpolarizes hippocampal CA1 and CA3 pyramidal cells through activation of GABAB postsynaptic receptors .
	manualset2
82830	4	397768	5	NULL	NULL	0	NULL	GABAB postsynaptic receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	GABA hyperpolarizes hippocampal CA1 and CA3 pyramidal cells through activation of GABAB postsynaptic receptors .
	manualset2
82831	1	397769	5	NULL	NULL	0	NULL	GABA levels	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	GABA levels in controls were 803 + / - 98 ( n = 7 ) and in demented patients 702 + / - 98 ( n = 7 ) pmol/ml .
	manualset2
82832	2	397769	5	NULL	NULL	0	NULL	controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	GABA levels in controls were 803 + / - 98 ( n = 7 ) and in demented patients 702 + / - 98 ( n = 7 ) pmol/ml .
	manualset2
82833	3	397769	5	NULL	NULL	0	NULL	803 + / - 98 ( n = 7 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	GABA levels in controls were 803 + / - 98 ( n = 7 ) and in demented patients 702 + / - 98 ( n = 7 ) pmol/ml .
	manualset2
82834	4	397769	5	NULL	NULL	0	NULL	demented patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	GABA levels in controls were 803 + / - 98 ( n = 7 ) and in demented patients 702 + / - 98 ( n = 7 ) pmol/ml .
	manualset2
82835	5	397769	5	NULL	NULL	0	NULL	702 + / - 98 ( n = 7 ) pmol/ml	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	GABA levels in controls were 803 + / - 98 ( n = 7 ) and in demented patients 702 + / - 98 ( n = 7 ) pmol/ml .
	manualset2
82836	1	397770	5	NULL	NULL	0	NULL	GABAB receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	GABAB receptors are abundant on dendritic spines , where they dampen postsynaptic excitability and inhibit Ca2 + influx through NMDA receptors when activated by spillover of GABA from neighboring GABAergic terminals .
	manualset2
82837	2	397770	5	NULL	NULL	0	NULL	dendritic spines	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	GABAB receptors are abundant on dendritic spines , where they dampen postsynaptic excitability and inhibit Ca2 + influx through NMDA receptors when activated by spillover of GABA from neighboring GABAergic terminals .
	manualset2
82838	3	397770	5	NULL	NULL	0	NULL	postsynaptic excitability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GABAB receptors are abundant on dendritic spines , where they dampen postsynaptic excitability and inhibit Ca2 + influx through NMDA receptors when activated by spillover of GABA from neighboring GABAergic terminals .
	manualset2
82839	4	397770	5	NULL	NULL	0	NULL	inhibit	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GABAB receptors are abundant on dendritic spines , where they dampen postsynaptic excitability and inhibit Ca2 + influx through NMDA receptors when activated by spillover of GABA from neighboring GABAergic terminals .
	manualset2
82840	5	397770	5	NULL	NULL	0	NULL	Ca2 + influx	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GABAB receptors are abundant on dendritic spines , where they dampen postsynaptic excitability and inhibit Ca2 + influx through NMDA receptors when activated by spillover of GABA from neighboring GABAergic terminals .
	manualset2
82841	6	397770	5	NULL	NULL	0	NULL	NMDA receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	GABAB receptors are abundant on dendritic spines , where they dampen postsynaptic excitability and inhibit Ca2 + influx through NMDA receptors when activated by spillover of GABA from neighboring GABAergic terminals .
	manualset2
82842	7	397770	5	NULL	NULL	0	NULL	spillover	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GABAB receptors are abundant on dendritic spines , where they dampen postsynaptic excitability and inhibit Ca2 + influx through NMDA receptors when activated by spillover of GABA from neighboring GABAergic terminals .
	manualset2
82843	8	397770	5	NULL	NULL	0	NULL	GABA	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	GABAB receptors are abundant on dendritic spines , where they dampen postsynaptic excitability and inhibit Ca2 + influx through NMDA receptors when activated by spillover of GABA from neighboring GABAergic terminals .
	manualset2
82844	9	397770	5	NULL	NULL	0	NULL	GABAergic terminals	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	GABAB receptors are abundant on dendritic spines , where they dampen postsynaptic excitability and inhibit Ca2 + influx through NMDA receptors when activated by spillover of GABA from neighboring GABAergic terminals .
	manualset2
82845	1	397771	5	NULL	NULL	0	NULL	GABAergic agents	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	GABAergic agents prevent alpha-melanocyte stimulating hormone induced anxiety and anorexia in rats .
	manualset2
82846	2	397771	5	NULL	NULL	NULL	NULL	alpha-melanocyte stimulating hormone	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	GABAergic agents prevent alpha-melanocyte stimulating hormone induced anxiety and anorexia in rats .
	manualset2
82847	3	397771	5	NULL	NULL	0	NULL	anxiety	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	GABAergic agents prevent alpha-melanocyte stimulating hormone induced anxiety and anorexia in rats .
	manualset2
82848	4	397771	5	NULL	NULL	0	NULL	anorexia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	GABAergic agents prevent alpha-melanocyte stimulating hormone induced anxiety and anorexia in rats .
	manualset2
82849	5	397771	5	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	GABAergic agents prevent alpha-melanocyte stimulating hormone induced anxiety and anorexia in rats .
	manualset2
82850	1	397772	5	NULL	NULL	0	NULL	GAD	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	GAD in beta-cells is associated with a vesicular compartment , similar to the GABA vesicles .
	manualset2
82851	2	397772	5	NULL	NULL	0	NULL	beta-cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	GAD in beta-cells is associated with a vesicular compartment , similar to the GABA vesicles .
	manualset2
82852	3	397772	5	NULL	NULL	0	NULL	vesicular compartment	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	GAD in beta-cells is associated with a vesicular compartment , similar to the GABA vesicles .
	manualset2
82853	4	397772	5	NULL	NULL	0	NULL	GABA vesicles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	GAD in beta-cells is associated with a vesicular compartment , similar to the GABA vesicles .
	manualset2
82854	1	397773	5	NULL	NULL	0	NULL	GAS	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	GAS was produced more copiously and more quickly by rostral PVN lesion than by lesion of the ventromedial ( VMH ) or dorsomedial ( DMH ) nucleus , and nearly as much by caudal PVN lesion .
	manualset2
82855	2	397773	5	NULL	NULL	0	NULL	rostral PVN lesion	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	GAS was produced more copiously and more quickly by rostral PVN lesion than by lesion of the ventromedial ( VMH ) or dorsomedial ( DMH ) nucleus , and nearly as much by caudal PVN lesion .
	manualset2
82856	3	397773	5	NULL	NULL	0	NULL	 lesion of the ventromedial ( VMH )	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	GAS was produced more copiously and more quickly by rostral PVN lesion than by lesion of the ventromedial ( VMH ) or dorsomedial ( DMH ) nucleus , and nearly as much by caudal PVN lesion .
	manualset2
82857	4	397773	5	NULL	NULL	0	NULL	dorsomedial ( DMH ) nucleus	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	GAS was produced more copiously and more quickly by rostral PVN lesion than by lesion of the ventromedial ( VMH ) or dorsomedial ( DMH ) nucleus , and nearly as much by caudal PVN lesion .
	manualset2
82858	5	397773	5	NULL	NULL	0	NULL	caudal PVN lesion	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	GAS was produced more copiously and more quickly by rostral PVN lesion than by lesion of the ventromedial ( VMH ) or dorsomedial ( DMH ) nucleus , and nearly as much by caudal PVN lesion .
	manualset2
82859	1	397774	5	NULL	NULL	0	NULL	GATA6 reporter gene	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	GATA6 reporter gene reveals myocardial phenotypic heterogeneity that is related to variations in gap junction coupling .
	manualset2
82860	2	397774	5	NULL	NULL	0	NULL	myocardial phenotypic heterogeneity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	GATA6 reporter gene reveals myocardial phenotypic heterogeneity that is related to variations in gap junction coupling .
	manualset2
82861	3	397774	5	NULL	NULL	0	NULL	gap junction coupling	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GATA6 reporter gene reveals myocardial phenotypic heterogeneity that is related to variations in gap junction coupling .
	manualset2
82862	1	397775	5	NULL	NULL	0	NULL	benign neoplasms of the parotid gland	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Several cases of benign neoplasms of the parotid gland ( excluding pleiomorphic adenomas ) ) .
	manualset2
82863	2	397775	5	NULL	NULL	0	NULL	pleiomorphic adenomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Several cases of benign neoplasms of the parotid gland ( excluding pleiomorphic adenomas ) ) .
	manualset2
82864	1	397776	5	NULL	NULL	0	NULL	GC number	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	GC number , proliferation , apoptosis , differentiation ( loss of OCT4 , DMRT1 expression , DMRT1 re-expression , GC migration ) and aggregation were evaluated at various foetal and postnatal ages .
	manualset2
82865	2	397776	5	NULL	NULL	0	NULL	proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GC number , proliferation , apoptosis , differentiation ( loss of OCT4 , DMRT1 expression , DMRT1 re-expression , GC migration ) and aggregation were evaluated at various foetal and postnatal ages .
	manualset2
82866	3	397776	5	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GC number , proliferation , apoptosis , differentiation ( loss of OCT4 , DMRT1 expression , DMRT1 re-expression , GC migration ) and aggregation were evaluated at various foetal and postnatal ages .
	manualset2
82867	4	397776	5	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GC number , proliferation , apoptosis , differentiation ( loss of OCT4 , DMRT1 expression , DMRT1 re-expression , GC migration ) and aggregation were evaluated at various foetal and postnatal ages .
	manualset2
82868	5	397776	5	NULL	NULL	0	NULL	loss of OCT4	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GC number , proliferation , apoptosis , differentiation ( loss of OCT4 , DMRT1 expression , DMRT1 re-expression , GC migration ) and aggregation were evaluated at various foetal and postnatal ages .
	manualset2
82869	6	397776	5	NULL	NULL	0	NULL	DMRT1 expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GC number , proliferation , apoptosis , differentiation ( loss of OCT4 , DMRT1 expression , DMRT1 re-expression , GC migration ) and aggregation were evaluated at various foetal and postnatal ages .
	manualset2
82870	7	397776	5	NULL	NULL	0	NULL	DMRT1 re-expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GC number , proliferation , apoptosis , differentiation ( loss of OCT4 , DMRT1 expression , DMRT1 re-expression , GC migration ) and aggregation were evaluated at various foetal and postnatal ages .
	manualset2
82871	8	397776	5	NULL	NULL	0	NULL	GC migration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GC number , proliferation , apoptosis , differentiation ( loss of OCT4 , DMRT1 expression , DMRT1 re-expression , GC migration ) and aggregation were evaluated at various foetal and postnatal ages .
	manualset2
82872	9	397776	5	NULL	NULL	0	NULL	aggregation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GC number , proliferation , apoptosis , differentiation ( loss of OCT4 , DMRT1 expression , DMRT1 re-expression , GC migration ) and aggregation were evaluated at various foetal and postnatal ages .
	manualset2
82873	10	397776	5	NULL	NULL	0	NULL	foetal and postnatal ages	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	GC number , proliferation , apoptosis , differentiation ( loss of OCT4 , DMRT1 expression , DMRT1 re-expression , GC migration ) and aggregation were evaluated at various foetal and postnatal ages .
	manualset2
82874	1	397777	5	NULL	NULL	0	NULL	GCN5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	GCN5 phosphorylated by activities in cellular extracts could be dephosphorylated by AtPP2C-6-6 in vitro .
	manualset2
82875	2	397777	5	NULL	NULL	0	NULL	cellular extracts	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	GCN5 phosphorylated by activities in cellular extracts could be dephosphorylated by AtPP2C-6-6 in vitro .
	manualset2
82876	3	397777	5	NULL	NULL	0	NULL	AtPP2C-6-6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	GCN5 phosphorylated by activities in cellular extracts could be dephosphorylated by AtPP2C-6-6 in vitro .
	manualset2
82877	1	397778	5	NULL	NULL	0	NULL	GC/MS systems	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	GC/MS systems are on the bench but still in the game .
	manualset2
82878	1	397779	5	NULL	NULL	0	NULL	GDC-0449 ( 25 and 50M )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	GDC-0449 ( 25 and 50M ) inhibited concentration-dependent cell growth in HCC and H1339 cells .
	manualset2
82879	2	397779	5	NULL	NULL	0	NULL	concentration-dependent cell growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GDC-0449 ( 25 and 50M ) inhibited concentration-dependent cell growth in HCC and H1339 cells .
	manualset2
82880	3	397779	5	NULL	NULL	0	NULL	HCC cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	GDC-0449 ( 25 and 50M ) inhibited concentration-dependent cell growth in HCC and H1339 cells .
	manualset2
82881	4	397779	5	NULL	NULL	0	NULL	H1339 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	GDC-0449 ( 25 and 50M ) inhibited concentration-dependent cell growth in HCC and H1339 cells .
	manualset2
82882	1	397780	5	NULL	NULL	0	NULL	GGA ( Golgi-localizing , gamma-adaptin ear homology domain , ARF-binding ) proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	GGA ( Golgi-localizing , gamma-adaptin ear homology domain , ARF-binding ) proteins are potential effectors of ADP-ribosylation factors , are associated with the trans-Golgi network ( TGN ) , and are involved in protein transport from this compartment .
	manualset2
82883	2	397780	5	NULL	NULL	0	NULL	potential effectors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	GGA ( Golgi-localizing , gamma-adaptin ear homology domain , ARF-binding ) proteins are potential effectors of ADP-ribosylation factors , are associated with the trans-Golgi network ( TGN ) , and are involved in protein transport from this compartment .
	manualset2
82884	3	397780	5	NULL	NULL	0	NULL	ADP-ribosylation factors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	GGA ( Golgi-localizing , gamma-adaptin ear homology domain , ARF-binding ) proteins are potential effectors of ADP-ribosylation factors , are associated with the trans-Golgi network ( TGN ) , and are involved in protein transport from this compartment .
	manualset2
82885	4	397780	5	NULL	NULL	0	NULL	trans-Golgi network ( TGN )	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	GGA ( Golgi-localizing , gamma-adaptin ear homology domain , ARF-binding ) proteins are potential effectors of ADP-ribosylation factors , are associated with the trans-Golgi network ( TGN ) , and are involved in protein transport from this compartment .
	manualset2
82886	5	397780	5	NULL	NULL	0	NULL	protein transport 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GGA ( Golgi-localizing , gamma-adaptin ear homology domain , ARF-binding ) proteins are potential effectors of ADP-ribosylation factors , are associated with the trans-Golgi network ( TGN ) , and are involved in protein transport from this compartment .
	manualset2
82887	6	397780	5	NULL	NULL	0	NULL	compartment	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	GGA ( Golgi-localizing , gamma-adaptin ear homology domain , ARF-binding ) proteins are potential effectors of ADP-ribosylation factors , are associated with the trans-Golgi network ( TGN ) , and are involved in protein transport from this compartment .
	manualset2
82888	1	397781	5	NULL	NULL	NULL	NULL	GI and SF AEs	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	GI and SF AEs were highest for subjects treated with ropinirole , while individuals treated with pramipexole exhibited the highest incidence of cognitive AEs .
	manualset2
82890	2	397781	5	NULL	NULL	NULL	NULL	subjects	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	GI and SF AEs were highest for subjects treated with ropinirole , while individuals treated with pramipexole exhibited the highest incidence of cognitive AEs .
	manualset2
82891	3	397781	5	NULL	NULL	NULL	NULL	ropinirole	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	GI and SF AEs were highest for subjects treated with ropinirole , while individuals treated with pramipexole exhibited the highest incidence of cognitive AEs .
	manualset2
82892	4	397781	5	NULL	NULL	NULL	NULL	individuals	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	GI and SF AEs were highest for subjects treated with ropinirole , while individuals treated with pramipexole exhibited the highest incidence of cognitive AEs .
	manualset2
82893	5	397781	5	NULL	NULL	NULL	NULL	pramipexole	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	GI and SF AEs were highest for subjects treated with ropinirole , while individuals treated with pramipexole exhibited the highest incidence of cognitive AEs .
	manualset2
82894	6	397781	5	NULL	NULL	0	NULL	cognitive AEs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	GI and SF AEs were highest for subjects treated with ropinirole , while individuals treated with pramipexole exhibited the highest incidence of cognitive AEs .
	manualset2
82895	1	397782	5	NULL	NULL	0	NULL	GLTP specificity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GLTP specificity encompasses both sphingoid - and glycerol-based glycolipids , but with a strict requirement that the initial sugar residue be beta-linked to the hydrophobic lipid backbone .
	manualset2
82896	2	397782	5	NULL	NULL	0	NULL	sphingoid - and glycerol-based glycolipids	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	GLTP specificity encompasses both sphingoid - and glycerol-based glycolipids , but with a strict requirement that the initial sugar residue be beta-linked to the hydrophobic lipid backbone .
	manualset2
82897	3	397782	5	NULL	NULL	0	NULL	sugar residue	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	GLTP specificity encompasses both sphingoid - and glycerol-based glycolipids , but with a strict requirement that the initial sugar residue be beta-linked to the hydrophobic lipid backbone .
	manualset2
82898	4	397782	5	NULL	NULL	0	NULL	hydrophobic lipid backbone	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	GLTP specificity encompasses both sphingoid - and glycerol-based glycolipids , but with a strict requirement that the initial sugar residue be beta-linked to the hydrophobic lipid backbone .
	manualset2
82899	1	397783	5	NULL	NULL	0	NULL	cellular immunity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Several indices of the state of cellular immunity in amyloidosis ( experimental-clinical study ) ) .
	manualset2
82900	2	397783	5	NULL	NULL	0	NULL	amyloidosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Several indices of the state of cellular immunity in amyloidosis ( experimental-clinical study ) ) .
	manualset2
82901	3	397783	5	NULL	NULL	0	NULL	experimental-clinical study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Several indices of the state of cellular immunity in amyloidosis ( experimental-clinical study ) ) .
	manualset2
82902	1	397784	5	NULL	NULL	0	NULL	GLU treatment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	GLU treatment caused time-dependent degeneration of outer hair cells ( OHCs ) in conjunction with a temporal increase of NOS activity in the organ of Corti .
	manualset2
82903	2	397784	5	NULL	NULL	0	NULL	time-dependent degeneration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GLU treatment caused time-dependent degeneration of outer hair cells ( OHCs ) in conjunction with a temporal increase of NOS activity in the organ of Corti .
	manualset2
82904	3	397784	5	NULL	NULL	0	NULL	outer hair cells ( OHCs )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	GLU treatment caused time-dependent degeneration of outer hair cells ( OHCs ) in conjunction with a temporal increase of NOS activity in the organ of Corti .
	manualset2
82905	4	397784	5	NULL	NULL	0	NULL	NOS activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GLU treatment caused time-dependent degeneration of outer hair cells ( OHCs ) in conjunction with a temporal increase of NOS activity in the organ of Corti .
	manualset2
82906	5	397784	5	NULL	NULL	0	NULL	organ of Corti	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	GLU treatment caused time-dependent degeneration of outer hair cells ( OHCs ) in conjunction with a temporal increase of NOS activity in the organ of Corti .
	manualset2
82907	1	397785	5	NULL	NULL	0	NULL	GLUT4 levels	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	GLUT4 levels were measured in whole membranes isolated from a variety of tissues in 4 and 20-week-old NZO and control NZC mice by Western blotting using a specific antibody to the C terminal end of the protein .
	manualset2
82908	2	397785	5	NULL	NULL	0	NULL	whole membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	GLUT4 levels were measured in whole membranes isolated from a variety of tissues in 4 and 20-week-old NZO and control NZC mice by Western blotting using a specific antibody to the C terminal end of the protein .
	manualset2
82909	3	397785	5	NULL	NULL	0	NULL	tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	GLUT4 levels were measured in whole membranes isolated from a variety of tissues in 4 and 20-week-old NZO and control NZC mice by Western blotting using a specific antibody to the C terminal end of the protein .
	manualset2
82910	4	397785	5	NULL	NULL	0	NULL	4 and 20-week-old NZO	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	GLUT4 levels were measured in whole membranes isolated from a variety of tissues in 4 and 20-week-old NZO and control NZC mice by Western blotting using a specific antibody to the C terminal end of the protein .
	manualset2
82911	5	397785	5	NULL	NULL	0	NULL	 control NZC mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	GLUT4 levels were measured in whole membranes isolated from a variety of tissues in 4 and 20-week-old NZO and control NZC mice by Western blotting using a specific antibody to the C terminal end of the protein .
	manualset2
82912	6	397785	5	NULL	NULL	0	NULL	Western blotting	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	GLUT4 levels were measured in whole membranes isolated from a variety of tissues in 4 and 20-week-old NZO and control NZC mice by Western blotting using a specific antibody to the C terminal end of the protein .
	manualset2
82913	7	397785	5	NULL	NULL	0	NULL	specific antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	GLUT4 levels were measured in whole membranes isolated from a variety of tissues in 4 and 20-week-old NZO and control NZC mice by Western blotting using a specific antibody to the C terminal end of the protein .
	manualset2
82914	8	397785	5	NULL	NULL	0	NULL	C terminal end	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	GLUT4 levels were measured in whole membranes isolated from a variety of tissues in 4 and 20-week-old NZO and control NZC mice by Western blotting using a specific antibody to the C terminal end of the protein .
	manualset2
82915	9	397785	5	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	GLUT4 levels were measured in whole membranes isolated from a variety of tissues in 4 and 20-week-old NZO and control NZC mice by Western blotting using a specific antibody to the C terminal end of the protein .
	manualset2
82916	1	397786	5	NULL	NULL	0	NULL	GPA	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	GPA was used as a biological cover for the following indications : problematic wound healing , 13 cases ; non-healing burns , 12 cases ; carcinoma , 4 cases ; unstable scar , 2 cases ; shortage of skin , 2 cases .
	manualset2
82917	2	397786	5	NULL	NULL	NULL	NULL	problematic wound healing	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	GPA was used as a biological cover for the following indications : problematic wound healing , 13 cases ; non-healing burns , 12 cases ; carcinoma , 4 cases ; unstable scar , 2 cases ; shortage of skin , 2 cases .
	manualset2
82918	3	397786	5	NULL	NULL	NULL	NULL	13 cases	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	GPA was used as a biological cover for the following indications : problematic wound healing , 13 cases ; non-healing burns , 12 cases ; carcinoma , 4 cases ; unstable scar , 2 cases ; shortage of skin , 2 cases .
	manualset2
82919	4	397786	5	NULL	NULL	0	NULL	non-healing burns	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	GPA was used as a biological cover for the following indications : problematic wound healing , 13 cases ; non-healing burns , 12 cases ; carcinoma , 4 cases ; unstable scar , 2 cases ; shortage of skin , 2 cases .
	manualset2
82920	5	397786	5	NULL	NULL	NULL	NULL	12 cases	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	GPA was used as a biological cover for the following indications : problematic wound healing , 13 cases ; non-healing burns , 12 cases ; carcinoma , 4 cases ; unstable scar , 2 cases ; shortage of skin , 2 cases .
	manualset2
82921	6	397786	5	NULL	NULL	0	NULL	carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	GPA was used as a biological cover for the following indications : problematic wound healing , 13 cases ; non-healing burns , 12 cases ; carcinoma , 4 cases ; unstable scar , 2 cases ; shortage of skin , 2 cases .
	manualset2
82922	7	397786	5	NULL	NULL	NULL	NULL	4 cases	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	GPA was used as a biological cover for the following indications : problematic wound healing , 13 cases ; non-healing burns , 12 cases ; carcinoma , 4 cases ; unstable scar , 2 cases ; shortage of skin , 2 cases .
	manualset2
82923	8	397786	5	NULL	NULL	0	NULL	unstable scar	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	GPA was used as a biological cover for the following indications : problematic wound healing , 13 cases ; non-healing burns , 12 cases ; carcinoma , 4 cases ; unstable scar , 2 cases ; shortage of skin , 2 cases .
	manualset2
82924	9	397786	5	NULL	NULL	NULL	NULL	2 cases	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	GPA was used as a biological cover for the following indications : problematic wound healing , 13 cases ; non-healing burns , 12 cases ; carcinoma , 4 cases ; unstable scar , 2 cases ; shortage of skin , 2 cases .
	manualset2
82925	10	397786	5	NULL	NULL	0	NULL	shortage of skin	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	GPA was used as a biological cover for the following indications : problematic wound healing , 13 cases ; non-healing burns , 12 cases ; carcinoma , 4 cases ; unstable scar , 2 cases ; shortage of skin , 2 cases .
	manualset2
82926	11	397786	5	NULL	NULL	NULL	NULL	2 cases	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	GPA was used as a biological cover for the following indications : problematic wound healing , 13 cases ; non-healing burns , 12 cases ; carcinoma , 4 cases ; unstable scar , 2 cases ; shortage of skin , 2 cases .
	manualset2
82927	1	397787	5	NULL	NULL	0	NULL	GPAT6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	GPAT6 is a member of the Arabidopsis GPAT family , which is crucial for cutin biosynthesis in sepals and petals .
	manualset2
82928	2	397787	5	NULL	NULL	0	NULL	member	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	GPAT6 is a member of the Arabidopsis GPAT family , which is crucial for cutin biosynthesis in sepals and petals .
	manualset2
82929	3	397787	5	NULL	NULL	0	NULL	Arabidopsis GPAT family	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	GPAT6 is a member of the Arabidopsis GPAT family , which is crucial for cutin biosynthesis in sepals and petals .
	manualset2
82930	4	397787	5	NULL	NULL	0	NULL	cutin biosynthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GPAT6 is a member of the Arabidopsis GPAT family , which is crucial for cutin biosynthesis in sepals and petals .
	manualset2
82931	5	397787	5	NULL	NULL	0	NULL	sepals	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	GPAT6 is a member of the Arabidopsis GPAT family , which is crucial for cutin biosynthesis in sepals and petals .
	manualset2
82932	6	397787	5	NULL	NULL	0	NULL	petals	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	GPAT6 is a member of the Arabidopsis GPAT family , which is crucial for cutin biosynthesis in sepals and petals .
	manualset2
82933	1	397788	5	NULL	NULL	0	NULL	GRFs	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	GRFs of the crush - injured animals showed earlier improvement compared to the experimental animals , whose overall GRF patterns failed to recover as well as the crush group .
	manualset2
82934	2	397788	5	NULL	NULL	0	NULL	crush - injured animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	GRFs of the crush - injured animals showed earlier improvement compared to the experimental animals , whose overall GRF patterns failed to recover as well as the crush group .
	manualset2
82935	3	397788	5	NULL	NULL	0	NULL	earlier improvement	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GRFs of the crush - injured animals showed earlier improvement compared to the experimental animals , whose overall GRF patterns failed to recover as well as the crush group .
	manualset2
82936	4	397788	5	NULL	NULL	0	NULL	experimental animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	GRFs of the crush - injured animals showed earlier improvement compared to the experimental animals , whose overall GRF patterns failed to recover as well as the crush group .
	manualset2
82937	5	397788	5	NULL	NULL	0	NULL	GRF patterns	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	GRFs of the crush - injured animals showed earlier improvement compared to the experimental animals , whose overall GRF patterns failed to recover as well as the crush group .
	manualset2
82938	6	397788	5	NULL	NULL	0	NULL	recover	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GRFs of the crush - injured animals showed earlier improvement compared to the experimental animals , whose overall GRF patterns failed to recover as well as the crush group .
	manualset2
82939	7	397788	5	NULL	NULL	0	NULL	crush group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	GRFs of the crush - injured animals showed earlier improvement compared to the experimental animals , whose overall GRF patterns failed to recover as well as the crush group .
	manualset2
82940	1	397789	5	NULL	NULL	0	NULL	GSK-3 beta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	GSK-3 beta , along with CDK5 , is responsible for most of the abnormal hyperphosphorylation of the microtubule-binding protein tau observed in Alzheimer 's disease .
	manualset2
82941	2	397789	5	NULL	NULL	0	NULL	CDK5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	GSK-3 beta , along with CDK5 , is responsible for most of the abnormal hyperphosphorylation of the microtubule-binding protein tau observed in Alzheimer 's disease .
	manualset2
82942	3	397789	5	NULL	NULL	0	NULL	abnormal hyperphosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GSK-3 beta , along with CDK5 , is responsible for most of the abnormal hyperphosphorylation of the microtubule-binding protein tau observed in Alzheimer 's disease .
	manualset2
82943	4	397789	5	NULL	NULL	0	NULL	microtubule-binding protein tau	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	GSK-3 beta , along with CDK5 , is responsible for most of the abnormal hyperphosphorylation of the microtubule-binding protein tau observed in Alzheimer 's disease .
	manualset2
82944	5	397789	5	NULL	NULL	0	NULL	Alzheimer 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	GSK-3 beta , along with CDK5 , is responsible for most of the abnormal hyperphosphorylation of the microtubule-binding protein tau observed in Alzheimer 's disease .
	manualset2
82945	1	397790	5	NULL	NULL	0	NULL	GSK232802A treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	GSK232802A treatment produced a small but sustained weight loss ( 4.6 1.0 % , P & lt ; 0.0001 ) and reduced adiposity ( P & lt ; 0.0001 ) , which was due at least in part to a suppression of food intake ( 3.6 3.7 % , P & lt ; 0.0001 ) .
	manualset2
82946	2	397790	5	NULL	NULL	NULL	NULL	sustained weight loss	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	GSK232802A treatment produced a small but sustained weight loss ( 4.6 1.0 % , P & lt ; 0.0001 ) and reduced adiposity ( P & lt ; 0.0001 ) , which was due at least in part to a suppression of food intake ( 3.6 3.7 % , P & lt ; 0.0001 ) .
	manualset2
82947	4	397790	5	NULL	NULL	NULL	NULL	reduced adiposity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	GSK232802A treatment produced a small but sustained weight loss ( 4.6 1.0 % , P & lt ; 0.0001 ) and reduced adiposity ( P & lt ; 0.0001 ) , which was due at least in part to a suppression of food intake ( 3.6 3.7 % , P & lt ; 0.0001 ) .
	manualset2
82948	6	397790	5	NULL	NULL	NULL	NULL	suppression	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	GSK232802A treatment produced a small but sustained weight loss ( 4.6 1.0 % , P & lt ; 0.0001 ) and reduced adiposity ( P & lt ; 0.0001 ) , which was due at least in part to a suppression of food intake ( 3.6 3.7 % , P & lt ; 0.0001 ) .
	manualset2
82949	7	397790	5	NULL	NULL	NULL	NULL	food intake	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	GSK232802A treatment produced a small but sustained weight loss ( 4.6 1.0 % , P & lt ; 0.0001 ) and reduced adiposity ( P & lt ; 0.0001 ) , which was due at least in part to a suppression of food intake ( 3.6 3.7 % , P & lt ; 0.0001 ) .
	manualset2
83170	3	397790	5	NULL	NULL	0	NULL	( 4.6 1.0 % , P & lt ; 0.0001 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	GSK232802A treatment produced a small but sustained weight loss ( 4.6 1.0 % , P & lt ; 0.0001 ) and reduced adiposity ( P & lt ; 0.0001 ) , which was due at least in part to a suppression of food intake ( 3.6 3.7 % , P & lt ; 0.0001 ) .
	manualset2
83171	5	397790	5	NULL	NULL	0	NULL	 ( P & lt ; 0.0001 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	GSK232802A treatment produced a small but sustained weight loss ( 4.6 1.0 % , P & lt ; 0.0001 ) and reduced adiposity ( P & lt ; 0.0001 ) , which was due at least in part to a suppression of food intake ( 3.6 3.7 % , P & lt ; 0.0001 ) .
	manualset2
83172	8	397790	5	NULL	NULL	0	NULL	 ( 3.6 3.7 % , P & lt ; 0.0001 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	GSK232802A treatment produced a small but sustained weight loss ( 4.6 1.0 % , P & lt ; 0.0001 ) and reduced adiposity ( P & lt ; 0.0001 ) , which was due at least in part to a suppression of food intake ( 3.6 3.7 % , P & lt ; 0.0001 ) .
	manualset2
82950	1	397791	5	NULL	NULL	0	NULL	GTN	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	GTN ( 1 mg sub-lingually ) had no significant effect on bleeding time 90-100 min following either placebo or GR32191B .
	manualset2
82951	2	397791	5	NULL	NULL	0	NULL	significant effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	GTN ( 1 mg sub-lingually ) had no significant effect on bleeding time 90-100 min following either placebo or GR32191B .
	manualset2
82952	3	397791	5	NULL	NULL	0	NULL	bleeding time 90-100 min	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	GTN ( 1 mg sub-lingually ) had no significant effect on bleeding time 90-100 min following either placebo or GR32191B .
	manualset2
82953	4	397791	5	NULL	NULL	0	NULL	placebo	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	GTN ( 1 mg sub-lingually ) had no significant effect on bleeding time 90-100 min following either placebo or GR32191B .
	manualset2
82954	5	397791	5	NULL	NULL	0	NULL	GR32191B	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	GTN ( 1 mg sub-lingually ) had no significant effect on bleeding time 90-100 min following either placebo or GR32191B .
	manualset2
82955	1	397792	5	NULL	NULL	0	NULL	GUS	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	GUS is required to degrade glycosaminoglycans ( GAGs ) , including heparan sulfate ( HS ) , dermatan sulfate ( DS ) , and chondroitin-4 , 6 - sulfate ( CS ) .
	manualset2
82956	2	397792	5	NULL	NULL	0	NULL	degrade	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GUS is required to degrade glycosaminoglycans ( GAGs ) , including heparan sulfate ( HS ) , dermatan sulfate ( DS ) , and chondroitin-4 , 6 - sulfate ( CS ) .
	manualset2
82957	3	397792	5	NULL	NULL	0	NULL	glycosaminoglycans ( GAGs )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	GUS is required to degrade glycosaminoglycans ( GAGs ) , including heparan sulfate ( HS ) , dermatan sulfate ( DS ) , and chondroitin-4 , 6 - sulfate ( CS ) .
	manualset2
82958	4	397792	5	NULL	NULL	0	NULL	heparan sulfate ( HS )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	GUS is required to degrade glycosaminoglycans ( GAGs ) , including heparan sulfate ( HS ) , dermatan sulfate ( DS ) , and chondroitin-4 , 6 - sulfate ( CS ) .
	manualset2
82959	5	397792	5	NULL	NULL	0	NULL	dermatan sulfate ( DS )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	GUS is required to degrade glycosaminoglycans ( GAGs ) , including heparan sulfate ( HS ) , dermatan sulfate ( DS ) , and chondroitin-4 , 6 - sulfate ( CS ) .
	manualset2
82960	6	397792	5	NULL	NULL	0	NULL	chondroitin-4 , 6 - sulfate ( CS )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	GUS is required to degrade glycosaminoglycans ( GAGs ) , including heparan sulfate ( HS ) , dermatan sulfate ( DS ) , and chondroitin-4 , 6 - sulfate ( CS ) .
	manualset2
82965	1	397794	5	NULL	NULL	0	NULL	GXMs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	GXMs from typical serotype A and serotype D isolates were excellent inhibitors of factor serum 3 .
	manualset2
82966	2	397794	5	NULL	NULL	0	NULL	typical serotype A	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	GXMs from typical serotype A and serotype D isolates were excellent inhibitors of factor serum 3 .
	manualset2
82967	3	397794	5	NULL	NULL	0	NULL	serotype D isolates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	GXMs from typical serotype A and serotype D isolates were excellent inhibitors of factor serum 3 .
	manualset2
82968	4	397794	5	NULL	NULL	NULL	NULL	excellent inhibitors	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	GXMs from typical serotype A and serotype D isolates were excellent inhibitors of factor serum 3 .
	manualset2
82969	5	397794	5	NULL	NULL	0	NULL	factor serum 3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	GXMs from typical serotype A and serotype D isolates were excellent inhibitors of factor serum 3 .
	manualset2
82970	1	397795	5	NULL	NULL	NULL	NULL	Gain - and loss-of-function analyses	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gain - and loss-of-function analyses show that sphingosine kinases affect trafficking of the G protein-coupled receptor Rhodopsin and the light-sensitive transient receptor potential ( TRP ) channel by modulating the levels of dihydrosphingosine 1 phosphate ( DHS1P ) and sphingosine 1 phosphate ( S1P ) .
	manualset2
82971	2	397795	5	NULL	NULL	0	NULL	sphingosine kinases	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Gain - and loss-of-function analyses show that sphingosine kinases affect trafficking of the G protein-coupled receptor Rhodopsin and the light-sensitive transient receptor potential ( TRP ) channel by modulating the levels of dihydrosphingosine 1 phosphate ( DHS1P ) and sphingosine 1 phosphate ( S1P ) .
	manualset2
82972	3	397795	5	NULL	NULL	0	NULL	 trafficking	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gain - and loss-of-function analyses show that sphingosine kinases affect trafficking of the G protein-coupled receptor Rhodopsin and the light-sensitive transient receptor potential ( TRP ) channel by modulating the levels of dihydrosphingosine 1 phosphate ( DHS1P ) and sphingosine 1 phosphate ( S1P ) .
	manualset2
82973	4	397795	5	NULL	NULL	0	NULL	G protein-coupled receptor Rhodopsin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Gain - and loss-of-function analyses show that sphingosine kinases affect trafficking of the G protein-coupled receptor Rhodopsin and the light-sensitive transient receptor potential ( TRP ) channel by modulating the levels of dihydrosphingosine 1 phosphate ( DHS1P ) and sphingosine 1 phosphate ( S1P ) .
	manualset2
82974	5	397795	5	NULL	NULL	0	NULL	light-sensitive transient receptor potential ( TRP ) channel	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Gain - and loss-of-function analyses show that sphingosine kinases affect trafficking of the G protein-coupled receptor Rhodopsin and the light-sensitive transient receptor potential ( TRP ) channel by modulating the levels of dihydrosphingosine 1 phosphate ( DHS1P ) and sphingosine 1 phosphate ( S1P ) .
	manualset2
82975	6	397795	5	NULL	NULL	0	NULL	dihydrosphingosine 1 phosphate ( DHS1P )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Gain - and loss-of-function analyses show that sphingosine kinases affect trafficking of the G protein-coupled receptor Rhodopsin and the light-sensitive transient receptor potential ( TRP ) channel by modulating the levels of dihydrosphingosine 1 phosphate ( DHS1P ) and sphingosine 1 phosphate ( S1P ) .
	manualset2
82976	7	397795	5	NULL	NULL	0	NULL	sphingosine 1 phosphate ( S1P )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Gain - and loss-of-function analyses show that sphingosine kinases affect trafficking of the G protein-coupled receptor Rhodopsin and the light-sensitive transient receptor potential ( TRP ) channel by modulating the levels of dihydrosphingosine 1 phosphate ( DHS1P ) and sphingosine 1 phosphate ( S1P ) .
	manualset2
83227	1	397796	5	NULL	NULL	0	NULL	cross-functional commitment	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gaining cross-functional commitment for a comprehensive PPE program not only will move the improvement process forward , but also will ensure the company benefits from optimal cost and performance advantages that positively impact the bottom line .
	manualset2
83228	2	397796	5	NULL	NULL	0	NULL	comprehensive PPE program	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Gaining cross-functional commitment for a comprehensive PPE program not only will move the improvement process forward , but also will ensure the company benefits from optimal cost and performance advantages that positively impact the bottom line .
	manualset2
83230	3	397796	5	NULL	NULL	0	NULL	improvement process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Gaining cross-functional commitment for a comprehensive PPE program not only will move the improvement process forward , but also will ensure the company benefits from optimal cost and performance advantages that positively impact the bottom line .
	manualset2
83231	4	397796	5	NULL	NULL	NULL	NULL	performance advantages	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gaining cross-functional commitment for a comprehensive PPE program not only will move the improvement process forward , but also will ensure the company benefits from optimal cost and performance advantages that positively impact the bottom line .
	manualset2
82977	1	397797	5	NULL	NULL	0	NULL	3p	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Gains of 3p were detected in 4/55 ( 7 % ) WDET , no WDEC , but notably in 3/6 ( 50 % ) PDEC ( OR 23.6 ; P = 0.003 ) .
	manualset2
82978	2	397797	5	NULL	NULL	0	NULL	4/55 ( 7 % ) WDET	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Gains of 3p were detected in 4/55 ( 7 % ) WDET , no WDEC , but notably in 3/6 ( 50 % ) PDEC ( OR 23.6 ; P = 0.003 ) .
	manualset2
82979	3	397797	5	NULL	NULL	0	NULL	WDEC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Gains of 3p were detected in 4/55 ( 7 % ) WDET , no WDEC , but notably in 3/6 ( 50 % ) PDEC ( OR 23.6 ; P = 0.003 ) .
	manualset2
82980	4	397797	5	NULL	NULL	0	NULL	3/6 ( 50 % ) PDEC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Gains of 3p were detected in 4/55 ( 7 % ) WDET , no WDEC , but notably in 3/6 ( 50 % ) PDEC ( OR 23.6 ; P = 0.003 ) .
	manualset2
82981	5	397797	5	NULL	NULL	0	NULL	23.6 ; P = 0.003	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Gains of 3p were detected in 4/55 ( 7 % ) WDET , no WDEC , but notably in 3/6 ( 50 % ) PDEC ( OR 23.6 ; P = 0.003 ) .
	manualset2
83173	1	397798	5	NULL	NULL	0	NULL	quicker bill collection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Gains outweigh costs of quicker bill collection .
	manualset2
82982	1	397799	5	NULL	NULL	0	NULL	Gal-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Gal-1 is up-regulated in hepatocarcinoma cells , although its role in liver pathophysiology remains uncertain .
	manualset2
82983	2	397799	5	NULL	NULL	0	NULL	hepatocarcinoma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Gal-1 is up-regulated in hepatocarcinoma cells , although its role in liver pathophysiology remains uncertain .
	manualset2
82984	3	397799	5	NULL	NULL	NULL	NULL	liver pathophysiology	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gal-1 is up-regulated in hepatocarcinoma cells , although its role in liver pathophysiology remains uncertain .
	manualset2
82985	1	397800	5	NULL	NULL	0	NULL	Galactorrhea	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Galactorrhea , oligo/amenorrhea , and hyperprolactinemia in patients with craniopharyngiomas .
	manualset2
82986	2	397800	5	NULL	NULL	0	NULL	oligo/amenorrhea	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Galactorrhea , oligo/amenorrhea , and hyperprolactinemia in patients with craniopharyngiomas .
	manualset2
82987	3	397800	5	NULL	NULL	0	NULL	hyperprolactinemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Galactorrhea , oligo/amenorrhea , and hyperprolactinemia in patients with craniopharyngiomas .
	manualset2
82988	4	397800	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Galactorrhea , oligo/amenorrhea , and hyperprolactinemia in patients with craniopharyngiomas .
	manualset2
82989	5	397800	5	NULL	NULL	0	NULL	craniopharyngiomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Galactorrhea , oligo/amenorrhea , and hyperprolactinemia in patients with craniopharyngiomas .
	manualset2
82990	1	397801	5	NULL	NULL	0	NULL	Gallbladder cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Gallbladder cancer and liver transplantation .
	manualset2
82991	2	397801	5	NULL	NULL	0	NULL	liver transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Gallbladder cancer and liver transplantation .
	manualset2
82992	1	397802	5	NULL	NULL	0	NULL	Gallbladder perforation	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Gallbladder perforation with contained empyema diagnosed by CT but missed by sonography and hepatobiliary scintigraphy .
	manualset2
82993	2	397802	5	NULL	NULL	0	NULL	contained empyema	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Gallbladder perforation with contained empyema diagnosed by CT but missed by sonography and hepatobiliary scintigraphy .
	manualset2
82994	3	397802	5	NULL	NULL	NULL	NULL	CT	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gallbladder perforation with contained empyema diagnosed by CT but missed by sonography and hepatobiliary scintigraphy .
	manualset2
82995	4	397802	5	NULL	NULL	0	NULL	sonography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Gallbladder perforation with contained empyema diagnosed by CT but missed by sonography and hepatobiliary scintigraphy .
	manualset2
82996	5	397802	5	NULL	NULL	0	NULL	hepatobiliary scintigraphy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Gallbladder perforation with contained empyema diagnosed by CT but missed by sonography and hepatobiliary scintigraphy .
	manualset2
82997	1	397803	5	NULL	NULL	0	NULL	Gambogenic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Gambogenic acid significantly inhibited cell proliferation and induced apoptosis .
	manualset2
82998	2	397803	5	NULL	NULL	0	NULL	cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gambogenic acid significantly inhibited cell proliferation and induced apoptosis .
	manualset2
82999	3	397803	5	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gambogenic acid significantly inhibited cell proliferation and induced apoptosis .
	manualset2
83000	1	397804	5	NULL	NULL	0	NULL	Gamma scintigraphic studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Gamma scintigraphic studies demonstrated that CaP capsules could pass through the stomach and small intestine intact and could release drug in colon .
	manualset2
83001	2	397804	5	NULL	NULL	0	NULL	CaP capsules	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Gamma scintigraphic studies demonstrated that CaP capsules could pass through the stomach and small intestine intact and could release drug in colon .
	manualset2
83002	3	397804	5	NULL	NULL	0	NULL	stomach	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Gamma scintigraphic studies demonstrated that CaP capsules could pass through the stomach and small intestine intact and could release drug in colon .
	manualset2
83003	4	397804	5	NULL	NULL	0	NULL	small intestine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Gamma scintigraphic studies demonstrated that CaP capsules could pass through the stomach and small intestine intact and could release drug in colon .
	manualset2
83004	5	397804	5	NULL	NULL	NULL	NULL	release	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gamma scintigraphic studies demonstrated that CaP capsules could pass through the stomach and small intestine intact and could release drug in colon .
	manualset2
83005	6	397804	5	NULL	NULL	0	NULL	drug	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Gamma scintigraphic studies demonstrated that CaP capsules could pass through the stomach and small intestine intact and could release drug in colon .
	manualset2
83006	7	397804	5	NULL	NULL	0	NULL	colon	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Gamma scintigraphic studies demonstrated that CaP capsules could pass through the stomach and small intestine intact and could release drug in colon .
	manualset2
83007	1	397805	5	NULL	NULL	0	NULL	Ganglioside pattern	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ganglioside pattern was altered only in the 2 month rats , showing a reduction of GM1 and GM1a in the synaptosomal fraction and of GD1a in the microsomal fraction .
	manualset2
83008	2	397805	5	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ganglioside pattern was altered only in the 2 month rats , showing a reduction of GM1 and GM1a in the synaptosomal fraction and of GD1a in the microsomal fraction .
	manualset2
83009	3	397805	5	NULL	NULL	0	NULL	GM1	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ganglioside pattern was altered only in the 2 month rats , showing a reduction of GM1 and GM1a in the synaptosomal fraction and of GD1a in the microsomal fraction .
	manualset2
83010	4	397805	5	NULL	NULL	0	NULL	GM1a	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ganglioside pattern was altered only in the 2 month rats , showing a reduction of GM1 and GM1a in the synaptosomal fraction and of GD1a in the microsomal fraction .
	manualset2
83011	5	397805	5	NULL	NULL	0	NULL	synaptosomal fraction	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Ganglioside pattern was altered only in the 2 month rats , showing a reduction of GM1 and GM1a in the synaptosomal fraction and of GD1a in the microsomal fraction .
	manualset2
83012	6	397805	5	NULL	NULL	0	NULL	GD1a	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ganglioside pattern was altered only in the 2 month rats , showing a reduction of GM1 and GM1a in the synaptosomal fraction and of GD1a in the microsomal fraction .
	manualset2
83013	7	397805	5	NULL	NULL	0	NULL	microsomal fraction	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Ganglioside pattern was altered only in the 2 month rats , showing a reduction of GM1 and GM1a in the synaptosomal fraction and of GD1a in the microsomal fraction .
	manualset2
83014	1	397806	5	NULL	NULL	NULL	NULL	Gap junctions	AnatomicalPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gap junctions appear among myocardiocytes , confirming the myogenic theory of heart contractions .
	manualset2
83015	2	397806	5	NULL	NULL	0	NULL	myocardiocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Gap junctions appear among myocardiocytes , confirming the myogenic theory of heart contractions .
	manualset2
83016	3	397806	5	NULL	NULL	0	NULL	myogenic theory of heart contractions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gap junctions appear among myocardiocytes , confirming the myogenic theory of heart contractions .
	manualset2
83017	1	397807	5	NULL	NULL	0	NULL	Gas-phase peptide sequencing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Gas-phase peptide sequencing by TEMPO-mediated radical generation .
	manualset2
83018	2	397807	5	NULL	NULL	NULL	NULL	TEMPO-mediated radical generation	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gas-phase peptide sequencing by TEMPO-mediated radical generation .
	manualset2
83019	1	397808	5	NULL	NULL	0	NULL	Gas-phase reactivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gas-phase reactivity of metavanadate ( VO3 ) - towards methanol and ethanol : experiment and theory .
	manualset2
83020	2	397808	5	NULL	NULL	0	NULL	metavanadate ( VO3 ) -	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Gas-phase reactivity of metavanadate ( VO3 ) - towards methanol and ethanol : experiment and theory .
	manualset2
83021	3	397808	5	NULL	NULL	0	NULL	methanol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Gas-phase reactivity of metavanadate ( VO3 ) - towards methanol and ethanol : experiment and theory .
	manualset2
83022	4	397808	5	NULL	NULL	0	NULL	ethanol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Gas-phase reactivity of metavanadate ( VO3 ) - towards methanol and ethanol : experiment and theory .
	manualset2
83023	5	397808	5	NULL	NULL	0	NULL	experiment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Gas-phase reactivity of metavanadate ( VO3 ) - towards methanol and ethanol : experiment and theory .
	manualset2
83024	6	397808	5	NULL	NULL	0	NULL	theory	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Gas-phase reactivity of metavanadate ( VO3 ) - towards methanol and ethanol : experiment and theory .
	manualset2
83025	1	397809	5	NULL	NULL	0	NULL	Gas	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Gas and solid sampling can be performed through the reactor bed with their composition profiles determined at steady state .
	manualset2
83026	2	397809	5	NULL	NULL	0	NULL	solid sampling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Gas and solid sampling can be performed through the reactor bed with their composition profiles determined at steady state .
	manualset2
83027	3	397809	5	NULL	NULL	0	NULL	reactor bed	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Gas and solid sampling can be performed through the reactor bed with their composition profiles determined at steady state .
	manualset2
83028	4	397809	5	NULL	NULL	0	NULL	composition profiles													NULL		0	NULL	NULL	NULL	NULL	NULL	Gas and solid sampling can be performed through the reactor bed with their composition profiles determined at steady state .
	manualset2
83029	1	397810	5	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Should we vaccinate children against influenza ? ) .
	manualset2
83030	2	397810	5	NULL	NULL	0	NULL	influenza	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Should we vaccinate children against influenza ? ) .
	manualset2
83031	1	397811	5	NULL	NULL	0	NULL	Gaseous environments	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Gaseous environments modify physiology in the brewing yeast Saccharomyces cerevisiae during batch alcoholic fermentation .
	manualset2
83032	2	397811	5	NULL	NULL	NULL	NULL	physiology	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gaseous environments modify physiology in the brewing yeast Saccharomyces cerevisiae during batch alcoholic fermentation .
	manualset2
83033	3	397811	5	NULL	NULL	0	NULL	brewing yeast Saccharomyces cerevisiae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Gaseous environments modify physiology in the brewing yeast Saccharomyces cerevisiae during batch alcoholic fermentation .
	manualset2
83034	4	397811	5	NULL	NULL	NULL	NULL	batch alcoholic fermentation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gaseous environments modify physiology in the brewing yeast Saccharomyces cerevisiae during batch alcoholic fermentation .
	manualset2
83037	1	397812	5	NULL	NULL	NULL	NULL	72 and 30 degrees F	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gasoline vehicles included normal particle mass ( particulate matter ( PM ) ) emitters ( tested at 72 and 30 degrees F ) , `` black '' and `` white '' smokers , and a new-technology vehicle ( tested at 72 degrees F ) .
	manualset2
83040	2	397812	5	NULL	NULL	NULL	NULL	72 degrees F	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gasoline vehicles included normal particle mass ( particulate matter ( PM ) ) emitters ( tested at 72 and 30 degrees F ) , `` black '' and `` white '' smokers , and a new-technology vehicle ( tested at 72 degrees F ) .
	manualset2
83041	1	397813	5	NULL	NULL	0	NULL	Gastric cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastric cancer is the second leading cause of cancer death worldwide .
	manualset2
83042	2	397813	5	NULL	NULL	0	NULL	cancer death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastric cancer is the second leading cause of cancer death worldwide .
	manualset2
83043	3	397813	5	NULL	NULL	0	NULL	worldwide	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastric cancer is the second leading cause of cancer death worldwide .
	manualset2
83044	1	397814	5	NULL	NULL	0	NULL	Gastric duplications	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastric duplications account for 2 % to 7 % of all gastrointestinal duplications .
	manualset2
83045	2	397814	5	NULL	NULL	0	NULL	2 % to 7 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastric duplications account for 2 % to 7 % of all gastrointestinal duplications .
	manualset2
83046	3	397814	5	NULL	NULL	0	NULL	gastrointestinal duplications	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastric duplications account for 2 % to 7 % of all gastrointestinal duplications .
	manualset2
83047	1	397815	5	NULL	NULL	0	NULL	Gastrin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrin and cholecystokinin levels in rats fed soya bean trypsin inhibitor .
	manualset2
83048	2	397815	5	NULL	NULL	0	NULL	cholecystokinin levels	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrin and cholecystokinin levels in rats fed soya bean trypsin inhibitor .
	manualset2
83049	3	397815	5	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrin and cholecystokinin levels in rats fed soya bean trypsin inhibitor .
	manualset2
83050	4	397815	5	NULL	NULL	0	NULL	soya bean trypsin inhibitor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrin and cholecystokinin levels in rats fed soya bean trypsin inhibitor .
	manualset2
83051	1	397816	5	NULL	NULL	0	NULL	Gastroccult reagent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastroccult reagent was used every 4 h to detect blood in gastric juice in 41 ICU patients at risk of GI bleeding ( GB ) and receiving antacid prophylaxis ( gastric pH greater than 3.5 ) .
	manualset2
83052	3	397816	5	NULL	NULL	NULL	NULL	blood	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gastroccult reagent was used every 4 h to detect blood in gastric juice in 41 ICU patients at risk of GI bleeding ( GB ) and receiving antacid prophylaxis ( gastric pH greater than 3.5 ) .
	manualset2
83053	4	397816	5	NULL	NULL	NULL	NULL	gastric juice	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gastroccult reagent was used every 4 h to detect blood in gastric juice in 41 ICU patients at risk of GI bleeding ( GB ) and receiving antacid prophylaxis ( gastric pH greater than 3.5 ) .
	manualset2
83054	5	397816	5	NULL	NULL	NULL	NULL	41 ICU patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gastroccult reagent was used every 4 h to detect blood in gastric juice in 41 ICU patients at risk of GI bleeding ( GB ) and receiving antacid prophylaxis ( gastric pH greater than 3.5 ) .
	manualset2
83055	6	397816	5	NULL	NULL	NULL	NULL	GI bleeding ( GB )	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gastroccult reagent was used every 4 h to detect blood in gastric juice in 41 ICU patients at risk of GI bleeding ( GB ) and receiving antacid prophylaxis ( gastric pH greater than 3.5 ) .
	manualset2
83056	7	397816	5	NULL	NULL	NULL	NULL	antacid prophylaxis	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gastroccult reagent was used every 4 h to detect blood in gastric juice in 41 ICU patients at risk of GI bleeding ( GB ) and receiving antacid prophylaxis ( gastric pH greater than 3.5 ) .
	manualset2
83057	8	397816	5	NULL	NULL	NULL	NULL	gastric pH greater than 3.5	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gastroccult reagent was used every 4 h to detect blood in gastric juice in 41 ICU patients at risk of GI bleeding ( GB ) and receiving antacid prophylaxis ( gastric pH greater than 3.5 ) .
	manualset2
83233	2	397816	5	NULL	NULL	NULL	NULL	every 4 h	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gastroccult reagent was used every 4 h to detect blood in gastric juice in 41 ICU patients at risk of GI bleeding ( GB ) and receiving antacid prophylaxis ( gastric pH greater than 3.5 ) .
	manualset2
83058	1	397817	5	NULL	NULL	0	NULL	Gastroenterologists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastroenterologists have , in spite of these facts , addressed this scientific field surprisingly late , in contrast to veterinarians , for whom the fermentative production of SCFAs has been acknowledged as a principal mechanism of intestinal digestion in plant-eating animals for decades .
	manualset2
83060	2	397817	5	NULL	NULL	0	NULL	veterinarians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastroenterologists have , in spite of these facts , addressed this scientific field surprisingly late , in contrast to veterinarians , for whom the fermentative production of SCFAs has been acknowledged as a principal mechanism of intestinal digestion in plant-eating animals for decades .
	manualset2
83061	3	397817	5	NULL	NULL	0	NULL	fermentative production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastroenterologists have , in spite of these facts , addressed this scientific field surprisingly late , in contrast to veterinarians , for whom the fermentative production of SCFAs has been acknowledged as a principal mechanism of intestinal digestion in plant-eating animals for decades .
	manualset2
83062	4	397817	5	NULL	NULL	0	NULL	SCFAs	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastroenterologists have , in spite of these facts , addressed this scientific field surprisingly late , in contrast to veterinarians , for whom the fermentative production of SCFAs has been acknowledged as a principal mechanism of intestinal digestion in plant-eating animals for decades .
	manualset2
83063	5	397817	5	NULL	NULL	0	NULL	principal mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastroenterologists have , in spite of these facts , addressed this scientific field surprisingly late , in contrast to veterinarians , for whom the fermentative production of SCFAs has been acknowledged as a principal mechanism of intestinal digestion in plant-eating animals for decades .
	manualset2
83064	6	397817	5	NULL	NULL	0	NULL	intestinal digestion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastroenterologists have , in spite of these facts , addressed this scientific field surprisingly late , in contrast to veterinarians , for whom the fermentative production of SCFAs has been acknowledged as a principal mechanism of intestinal digestion in plant-eating animals for decades .
	manualset2
83065	7	397817	5	NULL	NULL	0	NULL	plant-eating animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastroenterologists have , in spite of these facts , addressed this scientific field surprisingly late , in contrast to veterinarians , for whom the fermentative production of SCFAs has been acknowledged as a principal mechanism of intestinal digestion in plant-eating animals for decades .
	manualset2
83066	8	397817	5	NULL	NULL	0	NULL	decades	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastroenterologists have , in spite of these facts , addressed this scientific field surprisingly late , in contrast to veterinarians , for whom the fermentative production of SCFAs has been acknowledged as a principal mechanism of intestinal digestion in plant-eating animals for decades .
	manualset2
83067	1	397818	5	NULL	NULL	0	NULL	Gastrointestinal disease outcomes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrointestinal disease outcomes are also more severe , due to under-nutrition and lack of intervention strategies in these regions .
	manualset2
83068	2	397818	5	NULL	NULL	0	NULL	under-nutrition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrointestinal disease outcomes are also more severe , due to under-nutrition and lack of intervention strategies in these regions .
	manualset2
83069	3	397818	5	NULL	NULL	0	NULL	lack of intervention strategies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrointestinal disease outcomes are also more severe , due to under-nutrition and lack of intervention strategies in these regions .
	manualset2
83070	4	397818	5	NULL	NULL	0	NULL	regions	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrointestinal disease outcomes are also more severe , due to under-nutrition and lack of intervention strategies in these regions .
	manualset2
83071	1	397819	5	NULL	NULL	0	NULL	Sialolithiasis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Sialolithiasis of the parotid gland -- case report ) .
	manualset2
83072	2	397819	5	NULL	NULL	0	NULL	parotid gland	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Sialolithiasis of the parotid gland -- case report ) .
	manualset2
83174	3	397819	5	NULL	NULL	0	NULL	case report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Sialolithiasis of the parotid gland -- case report ) .
	manualset2
83074	1	397820	5	NULL	NULL	0	NULL	Gastrointestinal flora	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrointestinal flora and its alterations in critical illness .
	manualset2
83075	2	397820	5	NULL	NULL	0	NULL	critical illness	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrointestinal flora and its alterations in critical illness .
	manualset2
83076	1	397821	5	NULL	NULL	0	NULL	Gastrointestinal perforation	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrointestinal perforation early after peripheral blood stem cell transplantation for AL amyloidosis .
	manualset2
83077	2	397821	5	NULL	NULL	0	NULL	peripheral blood stem cell transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrointestinal perforation early after peripheral blood stem cell transplantation for AL amyloidosis .
	manualset2
83078	3	397821	5	NULL	NULL	0	NULL	AL amyloidosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrointestinal perforation early after peripheral blood stem cell transplantation for AL amyloidosis .
	manualset2
83079	1	397822	5	NULL	NULL	NULL	NULL	Gastrointestinal transit	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gastrointestinal transit of 14C-labeled nutrients was unchanged in hypophagic rats , suggesting a postabsorptive mechanism controlled the hypophagia .
	manualset2
83080	2	397822	5	NULL	NULL	0	NULL	14C-labeled nutrients	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrointestinal transit of 14C-labeled nutrients was unchanged in hypophagic rats , suggesting a postabsorptive mechanism controlled the hypophagia .
	manualset2
83081	3	397822	5	NULL	NULL	0	NULL	hypophagic rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrointestinal transit of 14C-labeled nutrients was unchanged in hypophagic rats , suggesting a postabsorptive mechanism controlled the hypophagia .
	manualset2
83082	4	397822	5	NULL	NULL	0	NULL	postabsorptive mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrointestinal transit of 14C-labeled nutrients was unchanged in hypophagic rats , suggesting a postabsorptive mechanism controlled the hypophagia .
	manualset2
83083	5	397822	5	NULL	NULL	0	NULL	hypophagia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrointestinal transit of 14C-labeled nutrients was unchanged in hypophagic rats , suggesting a postabsorptive mechanism controlled the hypophagia .
	manualset2
83084	1	397823	5	NULL	NULL	0	NULL	Gel filtration chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Gel filtration chromatography and sucrose gradient sedimentation studies indicate that in solution , native TnsB is a monomer of nonspherical shape .
	manualset2
83085	2	397823	5	NULL	NULL	0	NULL	sucrose gradient sedimentation studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Gel filtration chromatography and sucrose gradient sedimentation studies indicate that in solution , native TnsB is a monomer of nonspherical shape .
	manualset2
83086	3	397823	5	NULL	NULL	0	NULL	solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Gel filtration chromatography and sucrose gradient sedimentation studies indicate that in solution , native TnsB is a monomer of nonspherical shape .
	manualset2
83087	4	397823	5	NULL	NULL	0	NULL	native TnsB	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Gel filtration chromatography and sucrose gradient sedimentation studies indicate that in solution , native TnsB is a monomer of nonspherical shape .
	manualset2
83088	5	397823	5	NULL	NULL	0	NULL	monomer	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Gel filtration chromatography and sucrose gradient sedimentation studies indicate that in solution , native TnsB is a monomer of nonspherical shape .
	manualset2
83089	1	397824	5	NULL	NULL	0	NULL	efficient delivery	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Gelatin nanocarrier enables efficient delivery and phototoxicity of hypocrellin B against a mice tumor model .
	manualset2
83090	2	397824	5	NULL	NULL	0	NULL	phototoxicity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gelatin nanocarrier enables efficient delivery and phototoxicity of hypocrellin B against a mice tumor model .
	manualset2
83091	3	397824	5	NULL	NULL	0	NULL	hypocrellin B	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Gelatin nanocarrier enables efficient delivery and phototoxicity of hypocrellin B against a mice tumor model .
	manualset2
83092	4	397824	5	NULL	NULL	0	NULL	mice tumor model	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Gelatin nanocarrier enables efficient delivery and phototoxicity of hypocrellin B against a mice tumor model .
	manualset2
83093	1	397825	5	NULL	NULL	0	NULL	Geminin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Geminin prevents rereplication during xenopus development .
	manualset2
83094	2	397825	5	NULL	NULL	0	NULL	rereplication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Geminin prevents rereplication during xenopus development .
	manualset2
83095	3	397825	5	NULL	NULL	0	NULL	xenopus development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Geminin prevents rereplication during xenopus development .
	manualset2
83096	1	397826	5	NULL	NULL	0	NULL	children 's	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Gender labels and play styles : their relative contribution to children 's selection of playmates .
	manualset2
83097	2	397826	5	NULL	NULL	0	NULL	selection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gender labels and play styles : their relative contribution to children 's selection of playmates .
	manualset2
83098	3	397826	5	NULL	NULL	0	NULL	playmates	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Gender labels and play styles : their relative contribution to children 's selection of playmates .
	manualset2
83099	1	397827	5	NULL	NULL	0	NULL	iliac artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Sign of the iliac artery in patients with large gynecologic tumors ) .
	manualset2
83100	2	397827	5	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Sign of the iliac artery in patients with large gynecologic tumors ) .
	manualset2
83101	3	397827	5	NULL	NULL	0	NULL	large gynecologic tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Sign of the iliac artery in patients with large gynecologic tumors ) .
	manualset2
83102	1	397828	5	NULL	NULL	0	NULL	Gene arrays	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene arrays in lymphoma : Where will they fit in ?
	manualset2
83103	2	397828	5	NULL	NULL	0	NULL	lymphoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene arrays in lymphoma : Where will they fit in ?
	manualset2
83104	1	397829	5	NULL	NULL	0	NULL	Gene coexpression network topology	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene coexpression network topology of cardiac development , hypertrophy , and failure .
	manualset2
83105	2	397829	5	NULL	NULL	0	NULL	cardiac development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene coexpression network topology of cardiac development , hypertrophy , and failure .
	manualset2
83106	3	397829	5	NULL	NULL	NULL	NULL	hypertrophy	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene coexpression network topology of cardiac development , hypertrophy , and failure .
	manualset2
83107	4	397829	5	NULL	NULL	0	NULL	failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene coexpression network topology of cardiac development , hypertrophy , and failure .
	manualset2
83108	1	397830	5	NULL	NULL	0	NULL	Gene delivery	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene delivery of l-caldesmon protects cytoskeletal cell membrane integrity against adenovirus infection independently of myosin ATPase and actin assembly .
	manualset2
83109	2	397830	5	NULL	NULL	0	NULL	l-caldesmon	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene delivery of l-caldesmon protects cytoskeletal cell membrane integrity against adenovirus infection independently of myosin ATPase and actin assembly .
	manualset2
83110	3	397830	5	NULL	NULL	0	NULL	cytoskeletal cell membrane integrity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene delivery of l-caldesmon protects cytoskeletal cell membrane integrity against adenovirus infection independently of myosin ATPase and actin assembly .
	manualset2
83111	4	397830	5	NULL	NULL	0	NULL	adenovirus infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene delivery of l-caldesmon protects cytoskeletal cell membrane integrity against adenovirus infection independently of myosin ATPase and actin assembly .
	manualset2
83112	5	397830	5	NULL	NULL	0	NULL	myosin ATPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene delivery of l-caldesmon protects cytoskeletal cell membrane integrity against adenovirus infection independently of myosin ATPase and actin assembly .
	manualset2
83113	6	397830	5	NULL	NULL	0	NULL	actin assembly	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene delivery of l-caldesmon protects cytoskeletal cell membrane integrity against adenovirus infection independently of myosin ATPase and actin assembly .
	manualset2
82680	2	397831	14	13	NULL	NULL	NULL	poliovirion RNA	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene duplications in poliovirion RNA .
	manualset3
83115	1	397831	14	13	NULL	0	NULL	Gene duplications	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene duplications in poliovirion RNA .
	manualset3
82681	1	397832	14	13	NULL	NULL	NULL	real-time ( kinetic ) RT-PCR	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene expression analyses using real-time ( kinetic ) RT-PCR were performed to monitor the transcriptional evolution of EGFR ligands EGF , TGF , AR , BTC , EPI , NRG and HB-EGF in experimental modes induced to exhibit acquired resistance to the mono-HER1 inhibitor CTX , the mono-HER2 inhibitor trastuzumab ( Tzb ) or the dual HER1/HER2 inhibitor lapatinib ( LPT ) .
	manualset3
82682	2	397832	14	13	NULL	NULL	NULL	EGFR ligands	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene expression analyses using real-time ( kinetic ) RT-PCR were performed to monitor the transcriptional evolution of EGFR ligands EGF , TGF , AR , BTC , EPI , NRG and HB-EGF in experimental modes induced to exhibit acquired resistance to the mono-HER1 inhibitor CTX , the mono-HER2 inhibitor trastuzumab ( Tzb ) or the dual HER1/HER2 inhibitor lapatinib ( LPT ) .
	manualset3
82683	3	397832	14	13	NULL	0	NULL	EGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expression analyses using real-time ( kinetic ) RT-PCR were performed to monitor the transcriptional evolution of EGFR ligands EGF , TGF , AR , BTC , EPI , NRG and HB-EGF in experimental modes induced to exhibit acquired resistance to the mono-HER1 inhibitor CTX , the mono-HER2 inhibitor trastuzumab ( Tzb ) or the dual HER1/HER2 inhibitor lapatinib ( LPT ) .
	manualset3
82684	4	397832	14	13	NULL	0	NULL	TGF 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expression analyses using real-time ( kinetic ) RT-PCR were performed to monitor the transcriptional evolution of EGFR ligands EGF , TGF , AR , BTC , EPI , NRG and HB-EGF in experimental modes induced to exhibit acquired resistance to the mono-HER1 inhibitor CTX , the mono-HER2 inhibitor trastuzumab ( Tzb ) or the dual HER1/HER2 inhibitor lapatinib ( LPT ) .
	manualset3
82685	5	397832	14	13	NULL	0	NULL	AR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expression analyses using real-time ( kinetic ) RT-PCR were performed to monitor the transcriptional evolution of EGFR ligands EGF , TGF , AR , BTC , EPI , NRG and HB-EGF in experimental modes induced to exhibit acquired resistance to the mono-HER1 inhibitor CTX , the mono-HER2 inhibitor trastuzumab ( Tzb ) or the dual HER1/HER2 inhibitor lapatinib ( LPT ) .
	manualset3
82686	6	397832	14	13	NULL	0	NULL	BTC	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expression analyses using real-time ( kinetic ) RT-PCR were performed to monitor the transcriptional evolution of EGFR ligands EGF , TGF , AR , BTC , EPI , NRG and HB-EGF in experimental modes induced to exhibit acquired resistance to the mono-HER1 inhibitor CTX , the mono-HER2 inhibitor trastuzumab ( Tzb ) or the dual HER1/HER2 inhibitor lapatinib ( LPT ) .
	manualset3
82687	7	397832	14	13	NULL	0	NULL	EPI	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expression analyses using real-time ( kinetic ) RT-PCR were performed to monitor the transcriptional evolution of EGFR ligands EGF , TGF , AR , BTC , EPI , NRG and HB-EGF in experimental modes induced to exhibit acquired resistance to the mono-HER1 inhibitor CTX , the mono-HER2 inhibitor trastuzumab ( Tzb ) or the dual HER1/HER2 inhibitor lapatinib ( LPT ) .
	manualset3
82688	8	397832	14	13	NULL	0	NULL	NRG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expression analyses using real-time ( kinetic ) RT-PCR were performed to monitor the transcriptional evolution of EGFR ligands EGF , TGF , AR , BTC , EPI , NRG and HB-EGF in experimental modes induced to exhibit acquired resistance to the mono-HER1 inhibitor CTX , the mono-HER2 inhibitor trastuzumab ( Tzb ) or the dual HER1/HER2 inhibitor lapatinib ( LPT ) .
	manualset3
82689	9	397832	14	13	NULL	0	NULL	HB-EGF 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expression analyses using real-time ( kinetic ) RT-PCR were performed to monitor the transcriptional evolution of EGFR ligands EGF , TGF , AR , BTC , EPI , NRG and HB-EGF in experimental modes induced to exhibit acquired resistance to the mono-HER1 inhibitor CTX , the mono-HER2 inhibitor trastuzumab ( Tzb ) or the dual HER1/HER2 inhibitor lapatinib ( LPT ) .
	manualset3
82691	10	397832	14	13	NULL	NULL	NULL	mono-HER2 inhibitor trastuzumab ( Tzb ) 	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene expression analyses using real-time ( kinetic ) RT-PCR were performed to monitor the transcriptional evolution of EGFR ligands EGF , TGF , AR , BTC , EPI , NRG and HB-EGF in experimental modes induced to exhibit acquired resistance to the mono-HER1 inhibitor CTX , the mono-HER2 inhibitor trastuzumab ( Tzb ) or the dual HER1/HER2 inhibitor lapatinib ( LPT ) .
	manualset3
82692	11	397832	14	13	NULL	NULL	NULL	 mono-HER1 inhibitor CTX	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene expression analyses using real-time ( kinetic ) RT-PCR were performed to monitor the transcriptional evolution of EGFR ligands EGF , TGF , AR , BTC , EPI , NRG and HB-EGF in experimental modes induced to exhibit acquired resistance to the mono-HER1 inhibitor CTX , the mono-HER2 inhibitor trastuzumab ( Tzb ) or the dual HER1/HER2 inhibitor lapatinib ( LPT ) .
	manualset3
82696	12	397832	14	13	NULL	NULL	NULL	dual HER1/HER2 inhibitor lapatinib ( LPT ) 	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene expression analyses using real-time ( kinetic ) RT-PCR were performed to monitor the transcriptional evolution of EGFR ligands EGF , TGF , AR , BTC , EPI , NRG and HB-EGF in experimental modes induced to exhibit acquired resistance to the mono-HER1 inhibitor CTX , the mono-HER2 inhibitor trastuzumab ( Tzb ) or the dual HER1/HER2 inhibitor lapatinib ( LPT ) .
	manualset3
83116	13	397832	14	13	NULL	NULL	NULL	Gene expression analyses	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene expression analyses using real-time ( kinetic ) RT-PCR were performed to monitor the transcriptional evolution of EGFR ligands EGF , TGF , AR , BTC , EPI , NRG and HB-EGF in experimental modes induced to exhibit acquired resistance to the mono-HER1 inhibitor CTX , the mono-HER2 inhibitor trastuzumab ( Tzb ) or the dual HER1/HER2 inhibitor lapatinib ( LPT ) .
	manualset3
83117	14	397832	14	13	NULL	NULL	NULL	transcriptional evolution 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene expression analyses using real-time ( kinetic ) RT-PCR were performed to monitor the transcriptional evolution of EGFR ligands EGF , TGF , AR , BTC , EPI , NRG and HB-EGF in experimental modes induced to exhibit acquired resistance to the mono-HER1 inhibitor CTX , the mono-HER2 inhibitor trastuzumab ( Tzb ) or the dual HER1/HER2 inhibitor lapatinib ( LPT ) .
	manualset3
83118	15	397832	14	13	NULL	NULL	NULL	acquired resistance 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene expression analyses using real-time ( kinetic ) RT-PCR were performed to monitor the transcriptional evolution of EGFR ligands EGF , TGF , AR , BTC , EPI , NRG and HB-EGF in experimental modes induced to exhibit acquired resistance to the mono-HER1 inhibitor CTX , the mono-HER2 inhibitor trastuzumab ( Tzb ) or the dual HER1/HER2 inhibitor lapatinib ( LPT ) .
	manualset3
84551	16	397832	14	13	NULL	0	NULL	experimental modes 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expression analyses using real-time ( kinetic ) RT-PCR were performed to monitor the transcriptional evolution of EGFR ligands EGF , TGF , AR , BTC , EPI , NRG and HB-EGF in experimental modes induced to exhibit acquired resistance to the mono-HER1 inhibitor CTX , the mono-HER2 inhibitor trastuzumab ( Tzb ) or the dual HER1/HER2 inhibitor lapatinib ( LPT ) .
	manualset3
82698	1	397833	14	13	NULL	NULL	NULL	histone acetylation and methylation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene expression is controlled by epigenetic mechanisms such as histone acetylation and methylation , and recent studies have revealed that key developmental steps are regulated by the trimethylation of histone H3 lysine 4 ( H3K4me3 ) and lysine 27 ( H3K27me3 ) .
	manualset3
82701	2	397833	14	13	NULL	NULL	NULL	trimethylation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene expression is controlled by epigenetic mechanisms such as histone acetylation and methylation , and recent studies have revealed that key developmental steps are regulated by the trimethylation of histone H3 lysine 4 ( H3K4me3 ) and lysine 27 ( H3K27me3 ) .
	manualset3
82702	3	397833	14	13	NULL	NULL	NULL	histone H3 lysine 4	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene expression is controlled by epigenetic mechanisms such as histone acetylation and methylation , and recent studies have revealed that key developmental steps are regulated by the trimethylation of histone H3 lysine 4 ( H3K4me3 ) and lysine 27 ( H3K27me3 ) .
	manualset3
82703	4	397833	14	13	NULL	NULL	NULL	H3K4me3	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene expression is controlled by epigenetic mechanisms such as histone acetylation and methylation , and recent studies have revealed that key developmental steps are regulated by the trimethylation of histone H3 lysine 4 ( H3K4me3 ) and lysine 27 ( H3K27me3 ) .
	manualset3
82704	5	397833	14	13	NULL	NULL	NULL	lysine 27	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene expression is controlled by epigenetic mechanisms such as histone acetylation and methylation , and recent studies have revealed that key developmental steps are regulated by the trimethylation of histone H3 lysine 4 ( H3K4me3 ) and lysine 27 ( H3K27me3 ) .
	manualset3
82705	6	397833	14	13	NULL	NULL	NULL	H3K27me3	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene expression is controlled by epigenetic mechanisms such as histone acetylation and methylation , and recent studies have revealed that key developmental steps are regulated by the trimethylation of histone H3 lysine 4 ( H3K4me3 ) and lysine 27 ( H3K27me3 ) .
	manualset3
83119	7	397833	14	13	NULL	NULL	NULL	Gene expression 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene expression is controlled by epigenetic mechanisms such as histone acetylation and methylation , and recent studies have revealed that key developmental steps are regulated by the trimethylation of histone H3 lysine 4 ( H3K4me3 ) and lysine 27 ( H3K27me3 ) .
	manualset3
83120	8	397833	14	13	NULL	NULL	NULL	epigenetic mechanisms 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene expression is controlled by epigenetic mechanisms such as histone acetylation and methylation , and recent studies have revealed that key developmental steps are regulated by the trimethylation of histone H3 lysine 4 ( H3K4me3 ) and lysine 27 ( H3K27me3 ) .
	manualset3
83121	9	397833	14	13	NULL	NULL	NULL	key developmental steps	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene expression is controlled by epigenetic mechanisms such as histone acetylation and methylation , and recent studies have revealed that key developmental steps are regulated by the trimethylation of histone H3 lysine 4 ( H3K4me3 ) and lysine 27 ( H3K27me3 ) .
	manualset3
83122	10	397833	14	13	NULL	NULL	NULL	recent studies 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene expression is controlled by epigenetic mechanisms such as histone acetylation and methylation , and recent studies have revealed that key developmental steps are regulated by the trimethylation of histone H3 lysine 4 ( H3K4me3 ) and lysine 27 ( H3K27me3 ) .
	manualset3
82706	1	397834	14	13	NULL	0	NULL	CYP3A4	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expression of CYP3A4 , ABC-transporters ( MDR1 and MRP1-MRP5 ) and hPXR in three different human colon carcinoma cell lines .
	manualset3
82707	2	397834	14	13	NULL	0	NULL	MDR1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expression of CYP3A4 , ABC-transporters ( MDR1 and MRP1-MRP5 ) and hPXR in three different human colon carcinoma cell lines .
	manualset3
82708	3	397834	14	13	NULL	NULL	NULL	ABC-transporters	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene expression of CYP3A4 , ABC-transporters ( MDR1 and MRP1-MRP5 ) and hPXR in three different human colon carcinoma cell lines .
	manualset3
82709	4	397834	14	13	NULL	NULL	NULL	MRP1-MRP5	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene expression of CYP3A4 , ABC-transporters ( MDR1 and MRP1-MRP5 ) and hPXR in three different human colon carcinoma cell lines .
	manualset3
82711	6	397834	14	13	NULL	0	NULL	hPXR	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expression of CYP3A4 , ABC-transporters ( MDR1 and MRP1-MRP5 ) and hPXR in three different human colon carcinoma cell lines .
	manualset3
82712	7	397834	14	13	NULL	0	NULL	human colon carcinoma cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expression of CYP3A4 , ABC-transporters ( MDR1 and MRP1-MRP5 ) and hPXR in three different human colon carcinoma cell lines .
	manualset3
83123	8	397834	14	13	NULL	0	NULL	Gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expression of CYP3A4 , ABC-transporters ( MDR1 and MRP1-MRP5 ) and hPXR in three different human colon carcinoma cell lines .
	manualset3
82713	1	397835	14	13	NULL	0	NULL	S. cerevisiae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expression profiling and phenotype analyses of S. cerevisiae in response to changing copper reveals six genes with new roles in copper and iron metabolism .
	manualset3
82714	2	397835	14	13	NULL	NULL	NULL	Gene expression profiling 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene expression profiling and phenotype analyses of S. cerevisiae in response to changing copper reveals six genes with new roles in copper and iron metabolism .
	manualset3
82715	3	397835	14	13	NULL	NULL	NULL	phenotype analyses	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene expression profiling and phenotype analyses of S. cerevisiae in response to changing copper reveals six genes with new roles in copper and iron metabolism .
	manualset3
82716	4	397835	14	13	NULL	NULL	NULL	response to changing copper 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene expression profiling and phenotype analyses of S. cerevisiae in response to changing copper reveals six genes with new roles in copper and iron metabolism .
	manualset3
83124	5	397835	14	13	NULL	0	NULL	six genes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expression profiling and phenotype analyses of S. cerevisiae in response to changing copper reveals six genes with new roles in copper and iron metabolism .
	manualset3
83125	6	397835	14	13	NULL	0	NULL	copper and iron metabolism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expression profiling and phenotype analyses of S. cerevisiae in response to changing copper reveals six genes with new roles in copper and iron metabolism .
	manualset3
82717	1	397836	14	13	NULL	0	NULL	TH 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expressions of TH , GAD67 , and GluT1 were decreased , and those of TPH , beta-tubulin III , and S-100beta were increased by treatment with just ODNs , indicating the importance of the endogenous effect of HIF-1alpha on neuronal differentiation .
	manualset3
82718	2	397836	14	13	NULL	0	NULL	GAD67	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expressions of TH , GAD67 , and GluT1 were decreased , and those of TPH , beta-tubulin III , and S-100beta were increased by treatment with just ODNs , indicating the importance of the endogenous effect of HIF-1alpha on neuronal differentiation .
	manualset3
82719	3	397836	14	13	NULL	0	NULL	GluT1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expressions of TH , GAD67 , and GluT1 were decreased , and those of TPH , beta-tubulin III , and S-100beta were increased by treatment with just ODNs , indicating the importance of the endogenous effect of HIF-1alpha on neuronal differentiation .
	manualset3
82720	4	397836	14	13	NULL	0	NULL	TPH	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expressions of TH , GAD67 , and GluT1 were decreased , and those of TPH , beta-tubulin III , and S-100beta were increased by treatment with just ODNs , indicating the importance of the endogenous effect of HIF-1alpha on neuronal differentiation .
	manualset3
82721	5	397836	14	13	NULL	0	NULL	beta-tubulin III 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expressions of TH , GAD67 , and GluT1 were decreased , and those of TPH , beta-tubulin III , and S-100beta were increased by treatment with just ODNs , indicating the importance of the endogenous effect of HIF-1alpha on neuronal differentiation .
	manualset3
82722	6	397836	14	13	NULL	0	NULL	S-100beta	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expressions of TH , GAD67 , and GluT1 were decreased , and those of TPH , beta-tubulin III , and S-100beta were increased by treatment with just ODNs , indicating the importance of the endogenous effect of HIF-1alpha on neuronal differentiation .
	manualset3
82723	7	397836	14	13	NULL	NULL	NULL	treatment with just ODNs 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene expressions of TH , GAD67 , and GluT1 were decreased , and those of TPH , beta-tubulin III , and S-100beta were increased by treatment with just ODNs , indicating the importance of the endogenous effect of HIF-1alpha on neuronal differentiation .
	manualset3
82724	8	397836	14	13	NULL	0	NULL	HIF-1alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expressions of TH , GAD67 , and GluT1 were decreased , and those of TPH , beta-tubulin III , and S-100beta were increased by treatment with just ODNs , indicating the importance of the endogenous effect of HIF-1alpha on neuronal differentiation .
	manualset3
82725	9	397836	14	13	NULL	0	NULL	neuronal differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expressions of TH , GAD67 , and GluT1 were decreased , and those of TPH , beta-tubulin III , and S-100beta were increased by treatment with just ODNs , indicating the importance of the endogenous effect of HIF-1alpha on neuronal differentiation .
	manualset3
83126	10	397836	14	13	NULL	0	NULL	Gene expressions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expressions of TH , GAD67 , and GluT1 were decreased , and those of TPH , beta-tubulin III , and S-100beta were increased by treatment with just ODNs , indicating the importance of the endogenous effect of HIF-1alpha on neuronal differentiation .
	manualset3
83127	11	397836	14	13	NULL	0	NULL	endogenous effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expressions of TH , GAD67 , and GluT1 were decreased , and those of TPH , beta-tubulin III , and S-100beta were increased by treatment with just ODNs , indicating the importance of the endogenous effect of HIF-1alpha on neuronal differentiation .
	manualset3
82726	1	397837	14	13	NULL	NULL	NULL	partial pressure	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Significance of partial pressure of respiratory gas in the pulmonary alveoli and in arterial blood in respiratory function tests ; research in pulmonary tuberculosis ) .
	manualset3
82727	2	397837	14	13	NULL	0	NULL	pulmonary alveoli	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Significance of partial pressure of respiratory gas in the pulmonary alveoli and in arterial blood in respiratory function tests ; research in pulmonary tuberculosis ) .
	manualset3
82728	3	397837	14	13	NULL	0	NULL	arterial blood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Significance of partial pressure of respiratory gas in the pulmonary alveoli and in arterial blood in respiratory function tests ; research in pulmonary tuberculosis ) .
	manualset3
82729	4	397837	14	13	NULL	0	NULL	pulmonary tuberculosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Significance of partial pressure of respiratory gas in the pulmonary alveoli and in arterial blood in respiratory function tests ; research in pulmonary tuberculosis ) .
	manualset3
83128	5	397837	14	13	NULL	0	NULL	respiratory function tests	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Significance of partial pressure of respiratory gas in the pulmonary alveoli and in arterial blood in respiratory function tests ; research in pulmonary tuberculosis ) .
	manualset3
84552	6	397837	14	13	NULL	0	NULL	respiratory gas	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Significance of partial pressure of respiratory gas in the pulmonary alveoli and in arterial blood in respiratory function tests ; research in pulmonary tuberculosis ) .
	manualset3
82730	1	397838	14	13	NULL	0	NULL	X-gal staining	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expressions were visualized by both the quality of enzymatic color reaction using X-gal staining and by the quantification of the substrate chlorophenol red galactopyranoside ( CPRG ) in enucleated eyes on day 2 after gene transfer .
	manualset3
82731	2	397838	14	13	NULL	0	NULL	chlorophenol red galactopyranoside	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expressions were visualized by both the quality of enzymatic color reaction using X-gal staining and by the quantification of the substrate chlorophenol red galactopyranoside ( CPRG ) in enucleated eyes on day 2 after gene transfer .
	manualset3
82732	3	397838	14	13	NULL	0	NULL	CPRG	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expressions were visualized by both the quality of enzymatic color reaction using X-gal staining and by the quantification of the substrate chlorophenol red galactopyranoside ( CPRG ) in enucleated eyes on day 2 after gene transfer .
	manualset3
82733	4	397838	14	13	NULL	NULL	NULL	enucleated eyes	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene expressions were visualized by both the quality of enzymatic color reaction using X-gal staining and by the quantification of the substrate chlorophenol red galactopyranoside ( CPRG ) in enucleated eyes on day 2 after gene transfer .
	manualset3
82734	5	397838	14	13	NULL	NULL	NULL	on day 2 after gene transfer	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene expressions were visualized by both the quality of enzymatic color reaction using X-gal staining and by the quantification of the substrate chlorophenol red galactopyranoside ( CPRG ) in enucleated eyes on day 2 after gene transfer .
	manualset3
83129	6	397838	14	13	NULL	0	NULL	Gene expressions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expressions were visualized by both the quality of enzymatic color reaction using X-gal staining and by the quantification of the substrate chlorophenol red galactopyranoside ( CPRG ) in enucleated eyes on day 2 after gene transfer .
	manualset3
83130	7	397838	14	13	NULL	0	NULL	enzymatic color reaction 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expressions were visualized by both the quality of enzymatic color reaction using X-gal staining and by the quantification of the substrate chlorophenol red galactopyranoside ( CPRG ) in enucleated eyes on day 2 after gene transfer .
	manualset3
83131	8	397838	14	13	NULL	0	NULL	quantification of the substrate 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene expressions were visualized by both the quality of enzymatic color reaction using X-gal staining and by the quantification of the substrate chlorophenol red galactopyranoside ( CPRG ) in enucleated eyes on day 2 after gene transfer .
	manualset3
82735	1	397839	14	13	NULL	0	NULL	Gene therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene therapy : recent progress in the clinical oncology arena .
	manualset3
82736	2	397839	14	13	NULL	NULL	NULL	clinical oncology	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gene therapy : recent progress in the clinical oncology arena .
	manualset3
82737	1	397840	14	13	NULL	0	NULL	Gene therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene therapy for optic nerve disease .
	manualset3
82738	2	397840	14	13	NULL	0	NULL	optic nerve disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Gene therapy for optic nerve disease .
	manualset3
82739	1	397841	14	13	NULL	NULL	NULL	Genealogy	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genealogy of the spontaneously hypertensive rat and Wistar-Kyoto rat strains : implications for studies of inherited hypertension .
	manualset3
82740	2	397841	14	13	NULL	NULL	NULL	spontaneously hypertensive rat 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genealogy of the spontaneously hypertensive rat and Wistar-Kyoto rat strains : implications for studies of inherited hypertension .
	manualset3
82741	3	397841	14	13	NULL	0	NULL	Wistar-Kyoto rat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Genealogy of the spontaneously hypertensive rat and Wistar-Kyoto rat strains : implications for studies of inherited hypertension .
	manualset3
82742	4	397841	14	13	NULL	NULL	NULL	inherited hypertension	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genealogy of the spontaneously hypertensive rat and Wistar-Kyoto rat strains : implications for studies of inherited hypertension .
	manualset3
83132	5	397841	14	13	NULL	0	NULL	 implications for studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genealogy of the spontaneously hypertensive rat and Wistar-Kyoto rat strains : implications for studies of inherited hypertension .
	manualset3
83133	1	397842	14	13	NULL	0	NULL	General activation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	General activation of all major basal ganglia regions during locomotion is more likely to provide a dynamic background for cortical signal processing rather than to directly control precise movements .
	manualset3
83134	2	397842	14	13	NULL	0	NULL	all major basal ganglia regions	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	General activation of all major basal ganglia regions during locomotion is more likely to provide a dynamic background for cortical signal processing rather than to directly control precise movements .
	manualset3
83135	3	397842	14	13	NULL	0	NULL	 locomotion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	General activation of all major basal ganglia regions during locomotion is more likely to provide a dynamic background for cortical signal processing rather than to directly control precise movements .
	manualset3
83136	4	397842	14	13	NULL	0	NULL	cortical signal processing 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	General activation of all major basal ganglia regions during locomotion is more likely to provide a dynamic background for cortical signal processing rather than to directly control precise movements .
	manualset3
83137	5	397842	14	13	NULL	0	NULL	precise movements	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	General activation of all major basal ganglia regions during locomotion is more likely to provide a dynamic background for cortical signal processing rather than to directly control precise movements .
	manualset3
83138	1	397843	14	13	NULL	NULL	NULL	General vacuole index ( total vacuole number in a patient )	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	General vacuole index ( total vacuole number in a patient ) for left eyes was analyzed further .
	manualset3
83139	2	397843	14	13	NULL	0	NULL	left eyes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	General vacuole index ( total vacuole number in a patient ) for left eyes was analyzed further .
	manualset3
83140	1	397844	14	13	NULL	0	NULL	General practice	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	General practice : still waiting for green-paper .
	manualset3
83141	2	397844	14	13	NULL	0	NULL	green-paper	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	General practice : still waiting for green-paper .
	manualset3
83151	1	397846	14	13	NULL	NULL	NULL	General surgeon	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	General surgeon , biologist , professor .
	manualset3
83152	2	397846	14	13	NULL	0	NULL	biologist	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	General surgeon , biologist , professor .
	manualset3
83153	3	397846	14	13	NULL	0	NULL	professor 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	General surgeon , biologist , professor .
	manualset3
83154	1	397847	14	13	NULL	0	NULL	Generalizability analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Generalizability analyses suggest that while variability in PN ratings can be attributed to the choice of rater , candidate scores are reproducible over the 10-encounter CSA .
	manualset3
83155	2	397847	14	13	NULL	0	NULL	PN ratings	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Generalizability analyses suggest that while variability in PN ratings can be attributed to the choice of rater , candidate scores are reproducible over the 10-encounter CSA .
	manualset3
83156	3	397847	14	13	NULL	0	NULL	choice of rater	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Generalizability analyses suggest that while variability in PN ratings can be attributed to the choice of rater , candidate scores are reproducible over the 10-encounter CSA .
	manualset3
83157	4	397847	14	13	NULL	0	NULL	candidate scores	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Generalizability analyses suggest that while variability in PN ratings can be attributed to the choice of rater , candidate scores are reproducible over the 10-encounter CSA .
	manualset3
83158	5	397847	14	13	NULL	0	NULL	10-encounter CSA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Generalizability analyses suggest that while variability in PN ratings can be attributed to the choice of rater , candidate scores are reproducible over the 10-encounter CSA .
	manualset3
83159	1	397848	14	13	NULL	0	NULL	Silent myocardial infarction 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Silent myocardial infarction ) .
	manualset3
83160	1	397849	14	13	NULL	0	NULL	Generalized morphea	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Generalized morphea and lichen sclerosus et atrophicus successfully treated with sulphasalazine .
	manualset3
83161	2	397849	14	13	NULL	0	NULL	lichen sclerosus et atrophicus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Generalized morphea and lichen sclerosus et atrophicus successfully treated with sulphasalazine .
	manualset3
83163	3	397849	14	13	NULL	NULL	NULL	sulphasalazine	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Generalized morphea and lichen sclerosus et atrophicus successfully treated with sulphasalazine .
	manualset3
83164	1	397850	14	13	NULL	NULL	NULL	fetus	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Generally , in the fetus , FcR expression was lower than in the adult while in the neonate it approached values found later in life .
	manualset3
83165	2	397850	14	13	NULL	NULL	NULL	FcR expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Generally , in the fetus , FcR expression was lower than in the adult while in the neonate it approached values found later in life .
	manualset3
83166	3	397850	14	13	NULL	NULL	NULL	adult	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Generally , in the fetus , FcR expression was lower than in the adult while in the neonate it approached values found later in life .
	manualset3
83167	4	397850	14	13	NULL	NULL	NULL	neonate	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Generally , in the fetus , FcR expression was lower than in the adult while in the neonate it approached values found later in life .
	manualset3
83168	5	397850	14	13	NULL	0	NULL	approached values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Generally , in the fetus , FcR expression was lower than in the adult while in the neonate it approached values found later in life .
	manualset3
83169	6	397850	14	13	NULL	0	NULL	found later in life	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Generally , in the fetus , FcR expression was lower than in the adult while in the neonate it approached values found later in life .
	manualset3
83176	1	397851	14	13	NULL	NULL	NULL	retrogenes	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Generally , retrogenes emerge `` out of the testis , '' because they are often initially transcribed in testis and later evolve stronger and sometimes more diverse spatial expression patterns .
	manualset3
83177	2	397851	14	13	NULL	0	NULL	 out of the testis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Generally , retrogenes emerge `` out of the testis , '' because they are often initially transcribed in testis and later evolve stronger and sometimes more diverse spatial expression patterns .
	manualset3
83179	3	397851	14	13	NULL	NULL	NULL	testis	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Generally , retrogenes emerge `` out of the testis , '' because they are often initially transcribed in testis and later evolve stronger and sometimes more diverse spatial expression patterns .
	manualset3
83181	4	397851	14	13	NULL	NULL	NULL	sometimes more diverse spatial expression patterns	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Generally , retrogenes emerge `` out of the testis , '' because they are often initially transcribed in testis and later evolve stronger and sometimes more diverse spatial expression patterns .
	manualset3
83182	1	397852	14	13	NULL	0	NULL	time delay	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Generally speaking , time delay is a prevailing phenomenon in aquatic environments , since the production of allelopathic substance by competitive species is not instantaneous , but mediated by some time lag required for maturity of species .
	manualset3
83183	2	397852	14	13	NULL	0	NULL	aquatic environments	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Generally speaking , time delay is a prevailing phenomenon in aquatic environments , since the production of allelopathic substance by competitive species is not instantaneous , but mediated by some time lag required for maturity of species .
	manualset3
83184	3	397852	14	13	NULL	0	NULL	production of allelopathic substance 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Generally speaking , time delay is a prevailing phenomenon in aquatic environments , since the production of allelopathic substance by competitive species is not instantaneous , but mediated by some time lag required for maturity of species .
	manualset3
83185	4	397852	14	13	NULL	0	NULL	competitive species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Generally speaking , time delay is a prevailing phenomenon in aquatic environments , since the production of allelopathic substance by competitive species is not instantaneous , but mediated by some time lag required for maturity of species .
	manualset3
83186	5	397852	14	13	NULL	0	NULL	some time lag 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Generally speaking , time delay is a prevailing phenomenon in aquatic environments , since the production of allelopathic substance by competitive species is not instantaneous , but mediated by some time lag required for maturity of species .
	manualset3
83187	6	397852	14	13	NULL	0	NULL	maturity of species 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Generally speaking , time delay is a prevailing phenomenon in aquatic environments , since the production of allelopathic substance by competitive species is not instantaneous , but mediated by some time lag required for maturity of species .
	manualset3
83188	1	397853	14	13	NULL	NULL	NULL	total plate counts	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Generally speaking , total plate counts and lactic acid bacteria counts of all treatments slightly increased , with CHL being the lowest .
	manualset3
83189	2	397853	14	13	NULL	NULL	NULL	lactic acid bacteria counts	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Generally speaking , total plate counts and lactic acid bacteria counts of all treatments slightly increased , with CHL being the lowest .
	manualset3
83191	4	397853	14	13	NULL	0	NULL	CHL	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Generally speaking , total plate counts and lactic acid bacteria counts of all treatments slightly increased , with CHL being the lowest .
	manualset3
83192	3	397853	14	13	NULL	0	NULL	treatments	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Generally speaking , total plate counts and lactic acid bacteria counts of all treatments slightly increased , with CHL being the lowest .
	manualset3
83193	1	397854	14	13	NULL	0	NULL	Generation in vitro	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Generation in vitro of alloreactive lymphocytes is suppressed by the addition of spleen cells from mice infected with lymphocytic choriomeningitis virus .
	manualset3
83194	2	397854	14	13	NULL	0	NULL	alloreactive lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Generation in vitro of alloreactive lymphocytes is suppressed by the addition of spleen cells from mice infected with lymphocytic choriomeningitis virus .
	manualset3
83196	3	397854	14	13	NULL	NULL	NULL	spleen cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Generation in vitro of alloreactive lymphocytes is suppressed by the addition of spleen cells from mice infected with lymphocytic choriomeningitis virus .
	manualset3
83197	4	397854	14	13	NULL	NULL	NULL	mice infected 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Generation in vitro of alloreactive lymphocytes is suppressed by the addition of spleen cells from mice infected with lymphocytic choriomeningitis virus .
	manualset3
83199	5	397854	14	13	NULL	NULL	NULL	lymphocytic choriomeningitis virus	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Generation in vitro of alloreactive lymphocytes is suppressed by the addition of spleen cells from mice infected with lymphocytic choriomeningitis virus .
	manualset3
83200	1	397855	14	13	NULL	0	NULL	Generation of CTL	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Generation of CTL was accelerated in animals that had been previously primed in vivo by skin grafting .
	manualset3
83201	2	397855	14	13	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Generation of CTL was accelerated in animals that had been previously primed in vivo by skin grafting .
	manualset3
83203	3	397855	14	13	NULL	NULL	NULL	skin grafting	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Generation of CTL was accelerated in animals that had been previously primed in vivo by skin grafting .
	manualset3
83204	1	397856	14	13	NULL	0	NULL	Silicone elastomer prosthesis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Silicone elastomer prosthesis of the common bile duct .
	manualset3
83205	2	397856	14	13	NULL	0	NULL	common bile duct	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Silicone elastomer prosthesis of the common bile duct .
	manualset3
83206	1	397857	14	13	NULL	NULL	NULL	genetic engineering	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Generation of genetic engineering monoclonal antibodies against prion protein .
	manualset3
83207	2	397857	14	13	NULL	NULL	NULL	monoclonal antibodies	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Generation of genetic engineering monoclonal antibodies against prion protein .
	manualset3
83208	3	397857	14	13	NULL	0	NULL	prion protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Generation of genetic engineering monoclonal antibodies against prion protein .
	manualset3
83234	4	397857	14	13	NULL	0	NULL	Generation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Generation of genetic engineering monoclonal antibodies against prion protein .
	manualset3
83209	1	397858	14	13	NULL	NULL	NULL	new neurons	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Generation of new neurons is of particular interest because of the potential to treat diseases of the nervous system , such as neurodegenerative disorders and spinal cord injuries , with cell replacement therapy .
	manualset3
83210	2	397858	14	13	NULL	0	NULL	nervous system	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Generation of new neurons is of particular interest because of the potential to treat diseases of the nervous system , such as neurodegenerative disorders and spinal cord injuries , with cell replacement therapy .
	manualset3
83211	3	397858	14	13	NULL	NULL	NULL	neurodegenerative disorders	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Generation of new neurons is of particular interest because of the potential to treat diseases of the nervous system , such as neurodegenerative disorders and spinal cord injuries , with cell replacement therapy .
	manualset3
83212	4	397858	14	13	NULL	0	NULL	potential to treat diseases	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Generation of new neurons is of particular interest because of the potential to treat diseases of the nervous system , such as neurodegenerative disorders and spinal cord injuries , with cell replacement therapy .
	manualset3
83213	5	397858	14	13	NULL	0	NULL	spinal cord injuries	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Generation of new neurons is of particular interest because of the potential to treat diseases of the nervous system , such as neurodegenerative disorders and spinal cord injuries , with cell replacement therapy .
	manualset3
83214	6	397858	14	13	NULL	0	NULL	cell replacement therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Generation of new neurons is of particular interest because of the potential to treat diseases of the nervous system , such as neurodegenerative disorders and spinal cord injuries , with cell replacement therapy .
	manualset3
83235	7	397858	14	13	NULL	0	NULL	Generation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Generation of new neurons is of particular interest because of the potential to treat diseases of the nervous system , such as neurodegenerative disorders and spinal cord injuries , with cell replacement therapy .
	manualset3
83215	1	397859	14	13	NULL	NULL	NULL	Generation	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Generation of replication-competent and - defective HSV vectors .
	manualset3
83216	2	397859	14	13	NULL	0	NULL	replication-competent and - defective HSV vectors	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Generation of replication-competent and - defective HSV vectors .
	manualset3
83217	1	397860	14	13	NULL	NULL	NULL	Mitonyssoides stercoralis	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Generic and specific synonymy of Mitonyssoides stercoralis Yunker , Lukoschus , and Giesen , 1990 with Coprolactistus whitakeri Radovsky and Krantz , 1998 ( Acari : Mesostigmata : Macronyssidae ) .
	manualset3
83218	2	397860	14	13	NULL	0	NULL	Yunker	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Generic and specific synonymy of Mitonyssoides stercoralis Yunker , Lukoschus , and Giesen , 1990 with Coprolactistus whitakeri Radovsky and Krantz , 1998 ( Acari : Mesostigmata : Macronyssidae ) .
	manualset3
83219	3	397860	14	13	NULL	0	NULL	Lukoschus	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Generic and specific synonymy of Mitonyssoides stercoralis Yunker , Lukoschus , and Giesen , 1990 with Coprolactistus whitakeri Radovsky and Krantz , 1998 ( Acari : Mesostigmata : Macronyssidae ) .
	manualset3
83220	4	397860	14	13	NULL	0	NULL	Giesen	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Generic and specific synonymy of Mitonyssoides stercoralis Yunker , Lukoschus , and Giesen , 1990 with Coprolactistus whitakeri Radovsky and Krantz , 1998 ( Acari : Mesostigmata : Macronyssidae ) .
	manualset3
83221	5	397860	14	13	NULL	0	NULL	1990	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Generic and specific synonymy of Mitonyssoides stercoralis Yunker , Lukoschus , and Giesen , 1990 with Coprolactistus whitakeri Radovsky and Krantz , 1998 ( Acari : Mesostigmata : Macronyssidae ) .
	manualset3
83222	6	397860	14	13	NULL	0	NULL	Coprolactistus whitakeri	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Generic and specific synonymy of Mitonyssoides stercoralis Yunker , Lukoschus , and Giesen , 1990 with Coprolactistus whitakeri Radovsky and Krantz , 1998 ( Acari : Mesostigmata : Macronyssidae ) .
	manualset3
83223	7	397860	14	13	NULL	0	NULL	Radovsky	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Generic and specific synonymy of Mitonyssoides stercoralis Yunker , Lukoschus , and Giesen , 1990 with Coprolactistus whitakeri Radovsky and Krantz , 1998 ( Acari : Mesostigmata : Macronyssidae ) .
	manualset3
83224	8	397860	14	13	NULL	0	NULL	Krantz	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Generic and specific synonymy of Mitonyssoides stercoralis Yunker , Lukoschus , and Giesen , 1990 with Coprolactistus whitakeri Radovsky and Krantz , 1998 ( Acari : Mesostigmata : Macronyssidae ) .
	manualset3
83225	9	397860	14	13	NULL	0	NULL	1998 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Generic and specific synonymy of Mitonyssoides stercoralis Yunker , Lukoschus , and Giesen , 1990 with Coprolactistus whitakeri Radovsky and Krantz , 1998 ( Acari : Mesostigmata : Macronyssidae ) .
	manualset3
83226	10	397860	14	13	NULL	NULL	NULL	Acari : Mesostigmata : Macronyssidae	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Generic and specific synonymy of Mitonyssoides stercoralis Yunker , Lukoschus , and Giesen , 1990 with Coprolactistus whitakeri Radovsky and Krantz , 1998 ( Acari : Mesostigmata : Macronyssidae ) .
	manualset3
83236	1	397861	14	13	NULL	0	NULL	Genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Genes and development : molecular and logical themes .
	manualset3
83237	2	397861	14	13	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Genes and development : molecular and logical themes .
	manualset3
83238	3	397861	14	13	NULL	NULL	NULL	molecular and logical themes	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genes and development : molecular and logical themes .
	manualset3
83243	1	397863	14	13	NULL	0	NULL	Genes 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Genes encoding other potential virulence factors ( ace , efaA ( fs ) , ccf and cpd ) were frequently detected .
	manualset3
83244	2	397863	14	13	NULL	0	NULL	potential virulence factors	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Genes encoding other potential virulence factors ( ace , efaA ( fs ) , ccf and cpd ) were frequently detected .
	manualset3
83245	3	397863	14	13	NULL	0	NULL	ace	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Genes encoding other potential virulence factors ( ace , efaA ( fs ) , ccf and cpd ) were frequently detected .
	manualset3
83246	4	397863	14	13	NULL	0	NULL	efaA ( fs )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Genes encoding other potential virulence factors ( ace , efaA ( fs ) , ccf and cpd ) were frequently detected .
	manualset3
83247	5	397863	14	13	NULL	0	NULL	ccf	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Genes encoding other potential virulence factors ( ace , efaA ( fs ) , ccf and cpd ) were frequently detected .
	manualset3
83248	6	397863	14	13	NULL	0	NULL	cpd 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Genes encoding other potential virulence factors ( ace , efaA ( fs ) , ccf and cpd ) were frequently detected .
	manualset3
83249	1	397864	14	13	NULL	0	NULL	Genes 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Genes for the pathways involved in biological nitrogen fixation ( the nif gene cluster ) , nod genes including nodABC , and genes for the type III protein secretion system ( T3SS ) are present .
	manualset3
83250	2	397864	14	13	NULL	0	NULL	pathways 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Genes for the pathways involved in biological nitrogen fixation ( the nif gene cluster ) , nod genes including nodABC , and genes for the type III protein secretion system ( T3SS ) are present .
	manualset3
83251	3	397864	14	13	NULL	0	NULL	biological nitrogen fixation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Genes for the pathways involved in biological nitrogen fixation ( the nif gene cluster ) , nod genes including nodABC , and genes for the type III protein secretion system ( T3SS ) are present .
	manualset3
83252	4	397864	14	13	NULL	0	NULL	nif gene cluster	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Genes for the pathways involved in biological nitrogen fixation ( the nif gene cluster ) , nod genes including nodABC , and genes for the type III protein secretion system ( T3SS ) are present .
	manualset3
83253	5	397864	14	13	NULL	0	NULL	nod genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Genes for the pathways involved in biological nitrogen fixation ( the nif gene cluster ) , nod genes including nodABC , and genes for the type III protein secretion system ( T3SS ) are present .
	manualset3
83254	6	397864	14	13	NULL	0	NULL	nodABC	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Genes for the pathways involved in biological nitrogen fixation ( the nif gene cluster ) , nod genes including nodABC , and genes for the type III protein secretion system ( T3SS ) are present .
	manualset3
83255	7	397864	14	13	NULL	0	NULL	genes for the type III protein secretion system ( T3SS )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Genes for the pathways involved in biological nitrogen fixation ( the nif gene cluster ) , nod genes including nodABC , and genes for the type III protein secretion system ( T3SS ) are present .
	manualset3
83256	1	397865	14	13	NULL	NULL	NULL	Genetic components	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic , spatial , and temporal components of precise spawning synchrony in reef building corals of the Montastraea annularis species complex .
	manualset3
83257	2	397865	14	13	NULL	NULL	NULL	spatial components	GeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic , spatial , and temporal components of precise spawning synchrony in reef building corals of the Montastraea annularis species complex .
	manualset3
83258	3	397865	14	13	NULL	NULL	NULL	temporal components	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic , spatial , and temporal components of precise spawning synchrony in reef building corals of the Montastraea annularis species complex .
	manualset3
83259	4	397865	14	13	NULL	0	NULL	precise spawning synchrony	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic , spatial , and temporal components of precise spawning synchrony in reef building corals of the Montastraea annularis species complex .
	manualset3
83260	5	397865	14	13	NULL	0	NULL	reef building corals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic , spatial , and temporal components of precise spawning synchrony in reef building corals of the Montastraea annularis species complex .
	manualset3
83261	6	397865	14	13	NULL	0	NULL	Montastraea annularis species complex	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic , spatial , and temporal components of precise spawning synchrony in reef building corals of the Montastraea annularis species complex .
	manualset3
83262	1	397866	14	13	NULL	NULL	NULL	five active constitutents	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Simultaneous determination of five active constitutents in Xiaochaihu Tang by HPLC ) .
	manualset3
83263	2	397866	14	13	NULL	0	NULL	Xiaochaihu Tang 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	( Simultaneous determination of five active constitutents in Xiaochaihu Tang by HPLC ) .
	manualset3
83264	3	397866	14	13	NULL	0	NULL	HPLC	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Simultaneous determination of five active constitutents in Xiaochaihu Tang by HPLC ) .
	manualset3
83481	4	397866	14	13	NULL	0	NULL	 Simultaneous determination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Simultaneous determination of five active constitutents in Xiaochaihu Tang by HPLC ) .
	manualset3
83265	1	397867	14	13	NULL	0	NULL	Genetic ablation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic ablation of serum opacity factor ( SOF ) , a virulence determinant of S. pyogenes , reduced binding by approximately 50 % , and a recombinant peptide of SOF inhibited binding of fibulin-1 to streptococci by approximately 45 % .
	manualset3
83266	2	397867	14	13	NULL	0	NULL	serum opacity factor ( SOF )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic ablation of serum opacity factor ( SOF ) , a virulence determinant of S. pyogenes , reduced binding by approximately 50 % , and a recombinant peptide of SOF inhibited binding of fibulin-1 to streptococci by approximately 45 % .
	manualset3
83267	3	397867	14	13	NULL	NULL	NULL	a virulence determinant	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic ablation of serum opacity factor ( SOF ) , a virulence determinant of S. pyogenes , reduced binding by approximately 50 % , and a recombinant peptide of SOF inhibited binding of fibulin-1 to streptococci by approximately 45 % .
	manualset3
83268	4	397867	14	13	NULL	0	NULL	S. pyogenes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic ablation of serum opacity factor ( SOF ) , a virulence determinant of S. pyogenes , reduced binding by approximately 50 % , and a recombinant peptide of SOF inhibited binding of fibulin-1 to streptococci by approximately 45 % .
	manualset3
83270	5	397867	14	13	NULL	NULL	NULL	approximately 50 %	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic ablation of serum opacity factor ( SOF ) , a virulence determinant of S. pyogenes , reduced binding by approximately 50 % , and a recombinant peptide of SOF inhibited binding of fibulin-1 to streptococci by approximately 45 % .
	manualset3
83271	6	397867	14	13	NULL	NULL	NULL	recombinant peptide	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic ablation of serum opacity factor ( SOF ) , a virulence determinant of S. pyogenes , reduced binding by approximately 50 % , and a recombinant peptide of SOF inhibited binding of fibulin-1 to streptococci by approximately 45 % .
	manualset3
83272	7	397867	14	13	NULL	NULL	NULL	 SOF	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic ablation of serum opacity factor ( SOF ) , a virulence determinant of S. pyogenes , reduced binding by approximately 50 % , and a recombinant peptide of SOF inhibited binding of fibulin-1 to streptococci by approximately 45 % .
	manualset3
83274	8	397867	14	13	NULL	NULL	NULL	fibulin-1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic ablation of serum opacity factor ( SOF ) , a virulence determinant of S. pyogenes , reduced binding by approximately 50 % , and a recombinant peptide of SOF inhibited binding of fibulin-1 to streptococci by approximately 45 % .
	manualset3
83275	9	397867	14	13	NULL	NULL	NULL	streptococci 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic ablation of serum opacity factor ( SOF ) , a virulence determinant of S. pyogenes , reduced binding by approximately 50 % , and a recombinant peptide of SOF inhibited binding of fibulin-1 to streptococci by approximately 45 % .
	manualset3
83276	10	397867	14	13	NULL	NULL	NULL	approximately 45 % 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic ablation of serum opacity factor ( SOF ) , a virulence determinant of S. pyogenes , reduced binding by approximately 50 % , and a recombinant peptide of SOF inhibited binding of fibulin-1 to streptococci by approximately 45 % .
	manualset3
83277	1	397868	14	13	NULL	NULL	NULL	Genetic algorithm interval partial least squares regression 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic algorithm interval partial least squares regression combined successive projections algorithm for variable selection in near-infrared quantitative analysis of pigment in cucumber leaves .
	manualset3
83278	2	397868	14	13	NULL	NULL	NULL	successive projections algorithm	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic algorithm interval partial least squares regression combined successive projections algorithm for variable selection in near-infrared quantitative analysis of pigment in cucumber leaves .
	manualset3
83279	3	397868	14	13	NULL	0	NULL	variable selection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic algorithm interval partial least squares regression combined successive projections algorithm for variable selection in near-infrared quantitative analysis of pigment in cucumber leaves .
	manualset3
83280	4	397868	14	13	NULL	NULL	NULL	near-infrared quantitative analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic algorithm interval partial least squares regression combined successive projections algorithm for variable selection in near-infrared quantitative analysis of pigment in cucumber leaves .
	manualset3
83281	5	397868	14	13	NULL	0	NULL	pigment in cucumber leaves	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic algorithm interval partial least squares regression combined successive projections algorithm for variable selection in near-infrared quantitative analysis of pigment in cucumber leaves .
	manualset3
83282	1	397869	14	13	NULL	NULL	NULL	Genetic alterations	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic alterations in chromosome 10q24 .3 and glutathione S-transferase omega 2 gene polymorphism in ovarian cancer .
	manualset3
83283	2	397869	14	13	NULL	0	NULL	chromosome 10q24 .3	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic alterations in chromosome 10q24 .3 and glutathione S-transferase omega 2 gene polymorphism in ovarian cancer .
	manualset3
83285	3	397869	14	13	NULL	NULL	NULL	glutathione S-transferase omega 2 gene polymorphism	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic alterations in chromosome 10q24 .3 and glutathione S-transferase omega 2 gene polymorphism in ovarian cancer .
	manualset3
83286	4	397869	14	13	NULL	NULL	NULL	ovarian cancer	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic alterations in chromosome 10q24 .3 and glutathione S-transferase omega 2 gene polymorphism in ovarian cancer .
	manualset3
83287	1	397870	14	13	NULL	0	NULL	Genetic alterations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic alterations in chronic ulcerative colitis-associated adenoma-like DALMs are similar to non-colitic sporadic adenomas .
	manualset3
83288	2	397870	14	13	NULL	0	NULL	chronic ulcerative colitis-associated adenoma-like DALMs	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic alterations in chronic ulcerative colitis-associated adenoma-like DALMs are similar to non-colitic sporadic adenomas .
	manualset3
83289	3	397870	14	13	NULL	0	NULL	non-colitic sporadic adenomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic alterations in chronic ulcerative colitis-associated adenoma-like DALMs are similar to non-colitic sporadic adenomas .
	manualset3
83489	1	397871	14	13	NULL	0	NULL	Genetic analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic analyses in asthma : current concepts and future directions .
	manualset3
83490	2	397871	14	13	NULL	0	NULL	asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic analyses in asthma : current concepts and future directions .
	manualset3
83491	3	397871	14	13	NULL	0	NULL	current concepts	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic analyses in asthma : current concepts and future directions .
	manualset3
83493	4	397871	14	13	NULL	0	NULL	future directions	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic analyses in asthma : current concepts and future directions .
	manualset3
83501	1	397872	14	13	NULL	0	NULL	Genetic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic analysis in mice identifies cysteamine as a novel partner for artemisinin in the treatment of malaria .
	manualset3
83502	2	397872	14	13	NULL	0	NULL	 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic analysis in mice identifies cysteamine as a novel partner for artemisinin in the treatment of malaria .
	manualset3
83504	3	397872	14	13	NULL	0	NULL	 cysteamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic analysis in mice identifies cysteamine as a novel partner for artemisinin in the treatment of malaria .
	manualset3
83507	4	397872	14	13	NULL	0	NULL	artemisinin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic analysis in mice identifies cysteamine as a novel partner for artemisinin in the treatment of malaria .
	manualset3
83510	5	397872	14	13	NULL	NULL	NULL	malaria	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic analysis in mice identifies cysteamine as a novel partner for artemisinin in the treatment of malaria .
	manualset3
83600	6	397872	14	13	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic analysis in mice identifies cysteamine as a novel partner for artemisinin in the treatment of malaria .
	manualset3
83512	1	397873	14	13	NULL	0	NULL	Genetic analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic analysis indicated that the cfiA gene was present in some but not all of the isolates with high MICs to the carbapenems .
	manualset3
83513	2	397873	14	13	NULL	0	NULL	cfiA gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic analysis indicated that the cfiA gene was present in some but not all of the isolates with high MICs to the carbapenems .
	manualset3
83523	3	397873	14	13	NULL	0	NULL	isolates	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic analysis indicated that the cfiA gene was present in some but not all of the isolates with high MICs to the carbapenems .
	manualset3
83525	4	397873	14	13	NULL	NULL	NULL	high MICs	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic analysis indicated that the cfiA gene was present in some but not all of the isolates with high MICs to the carbapenems .
	manualset3
83527	5	397873	14	13	NULL	0	NULL	carbapenems 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic analysis indicated that the cfiA gene was present in some but not all of the isolates with high MICs to the carbapenems .
	manualset3
83536	1	397874	14	13	NULL	0	NULL	Genetic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic analysis of the additional sex combs locus of Drosophila melanogaster .
	manualset3
83546	2	397874	14	13	NULL	NULL	NULL	additional sex combs locus	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic analysis of the additional sex combs locus of Drosophila melanogaster .
	manualset3
83547	3	397874	14	13	NULL	0	NULL	Drosophila melanogaster	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic analysis of the additional sex combs locus of Drosophila melanogaster .
	manualset3
83551	1	397875	14	13	NULL	0	NULL	Genetic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic analysis of turbot pathogenic Streptococcus parauberis strains by ribotyping and random amplified polymorphic DNA .
	manualset3
83555	1	397875	14	13	NULL	0	NULL	turbot pathogenic Streptococcus parauberis strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic analysis of turbot pathogenic Streptococcus parauberis strains by ribotyping and random amplified polymorphic DNA .
	manualset3
83556	3	397875	14	13	NULL	0	NULL	ribotyping	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic analysis of turbot pathogenic Streptococcus parauberis strains by ribotyping and random amplified polymorphic DNA .
	manualset3
83558	4	397875	14	13	NULL	0	NULL	random amplified polymorphic DNA 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic analysis of turbot pathogenic Streptococcus parauberis strains by ribotyping and random amplified polymorphic DNA .
	manualset3
83561	1	397876	14	13	NULL	0	NULL	Genetic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic analysis that reveals a monoclonal T-cell population is also relevant .
	manualset3
83564	2	397876	14	13	NULL	0	NULL	monoclonal T-cell population 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic analysis that reveals a monoclonal T-cell population is also relevant .
	manualset3
83569	1	397877	14	13	NULL	0	NULL	Simultaneous occurrence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Simultaneous occurrence of excessive myopic fundus changes , cataract , corneal opacity and elastoma diffusum Dubreuilh ) .
	manualset3
83572	2	397877	14	13	NULL	NULL	NULL	excessive myopic fundus changes 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Simultaneous occurrence of excessive myopic fundus changes , cataract , corneal opacity and elastoma diffusum Dubreuilh ) .
	manualset3
83574	3	397877	14	13	NULL	0	NULL	cataract	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Simultaneous occurrence of excessive myopic fundus changes , cataract , corneal opacity and elastoma diffusum Dubreuilh ) .
	manualset3
83577	4	397877	14	13	NULL	NULL	NULL	corneal opacity	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Simultaneous occurrence of excessive myopic fundus changes , cataract , corneal opacity and elastoma diffusum Dubreuilh ) .
	manualset3
83578	5	397877	14	13	NULL	0	NULL	elastoma diffusum	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Simultaneous occurrence of excessive myopic fundus changes , cataract , corneal opacity and elastoma diffusum Dubreuilh ) .
	manualset3
83579	6	397877	14	13	NULL	0	NULL	Dubreuilh 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( Simultaneous occurrence of excessive myopic fundus changes , cataract , corneal opacity and elastoma diffusum Dubreuilh ) .
	manualset3
83582	3	397878	14	13	NULL	0	NULL	thymidine-dependent mutants of pneumococcus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic and biochemical properties of thymidine-dependent mutants of pneumococcus .
	manualset3
83583	1	397879	14	13	NULL	0	NULL	Genetic study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic and functional study of the IPO5 gene in schizophrenia .
	manualset3
83584	2	397879	14	13	NULL	0	NULL	functional study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic and functional study of the IPO5 gene in schizophrenia .
	manualset3
83585	3	397879	14	13	NULL	0	NULL	 IPO5 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic and functional study of the IPO5 gene in schizophrenia .
	manualset3
83586	4	397879	14	13	NULL	0	NULL	schizophrenia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic and functional study of the IPO5 gene in schizophrenia .
	manualset3
83589	1	397880	14	13	NULL	0	NULL	Genetic studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic and molecular genetic studies in the diagnosis of myeloid diseases .
	manualset3
83590	2	397880	14	13	NULL	NULL	NULL	molecular genetic studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic and molecular genetic studies in the diagnosis of myeloid diseases .
	manualset3
83592	3	397880	14	13	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic and molecular genetic studies in the diagnosis of myeloid diseases .
	manualset3
83593	4	397880	14	13	NULL	0	NULL	myeloid diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic and molecular genetic studies in the diagnosis of myeloid diseases .
	manualset3
83994	1	397881	14	13	NULL	0	NULL	Genetic animal models	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic animal models : focus on schizophrenia .
	manualset3
83995	2	397881	14	13	NULL	0	NULL	schizophrenia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic animal models : focus on schizophrenia .
	manualset3
83996	1	397882	14	13	NULL	0	NULL	Genetic characterisation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic characterisation of six Sarcocystis species from reindeer ( Rangifer tarandus tarandus ) in Norway based on the small subunit rRNA gene .
	manualset3
83997	2	397882	14	13	NULL	0	NULL	six	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic characterisation of six Sarcocystis species from reindeer ( Rangifer tarandus tarandus ) in Norway based on the small subunit rRNA gene .
	manualset3
83998	3	397882	14	13	NULL	0	NULL	Sarcocystis species 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic characterisation of six Sarcocystis species from reindeer ( Rangifer tarandus tarandus ) in Norway based on the small subunit rRNA gene .
	manualset3
83999	4	397882	14	13	NULL	0	NULL	reindeer ( Rangifer tarandus tarandus )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic characterisation of six Sarcocystis species from reindeer ( Rangifer tarandus tarandus ) in Norway based on the small subunit rRNA gene .
	manualset3
84000	5	397882	14	13	NULL	0	NULL	Norway	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic characterisation of six Sarcocystis species from reindeer ( Rangifer tarandus tarandus ) in Norway based on the small subunit rRNA gene .
	manualset3
84001	6	397882	14	13	NULL	0	NULL	small subunit rRNA gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic characterisation of six Sarcocystis species from reindeer ( Rangifer tarandus tarandus ) in Norway based on the small subunit rRNA gene .
	manualset3
84002	1	397883	14	13	NULL	0	NULL	Genetic characterization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic characterization of equine arteritis virus during persistent infection of stallions .
	manualset3
84003	2	397883	14	13	NULL	0	NULL	equine arteritis virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic characterization of equine arteritis virus during persistent infection of stallions .
	manualset3
84004	3	397883	14	13	NULL	0	NULL	persistent infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic characterization of equine arteritis virus during persistent infection of stallions .
	manualset3
84005	4	397883	14	13	NULL	0	NULL	stallions	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic characterization of equine arteritis virus during persistent infection of stallions .
	manualset3
84006	1	397884	14	13	NULL	0	NULL	Genetic data	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic data suggest that Stp1 acts either at , or above , the level of Ras2 , possibly on the Ira proteins .
	manualset3
84007	2	397884	14	13	NULL	NULL	NULL	 Stp1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic data suggest that Stp1 acts either at , or above , the level of Ras2 , possibly on the Ira proteins .
	manualset3
84008	3	397884	14	13	NULL	NULL	NULL	Ras2 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic data suggest that Stp1 acts either at , or above , the level of Ras2 , possibly on the Ira proteins .
	manualset3
84009	3	397884	14	13	NULL	0	NULL	Ira proteins 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic data suggest that Stp1 acts either at , or above , the level of Ras2 , possibly on the Ira proteins .
	manualset3
84010	1	397885	14	13	NULL	0	NULL	Single-dose 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( Single-dose and high-volume Bretschneider cardioplegic solution for congenital heart surgery ) .
	manualset3
84011	2	397885	14	13	NULL	0	NULL	high-volume 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( Single-dose and high-volume Bretschneider cardioplegic solution for congenital heart surgery ) .
	manualset3
84012	3	397885	14	13	NULL	0	NULL	Bretschneider cardioplegic solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Single-dose and high-volume Bretschneider cardioplegic solution for congenital heart surgery ) .
	manualset3
84013	4	397885	14	13	NULL	0	NULL	congenital heart surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Single-dose and high-volume Bretschneider cardioplegic solution for congenital heart surgery ) .
	manualset3
84014	1	397886	14	13	NULL	NULL	NULL	Genetic differentiation 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic differentiation was highest between BC and the South Cascades , and intermediate between BC and the North Cascades .
	manualset3
84015	2	397886	14	13	NULL	NULL	NULL	BC	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic differentiation was highest between BC and the South Cascades , and intermediate between BC and the North Cascades .
	manualset3
84016	3	397886	14	13	NULL	0	NULL	South Cascades	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic differentiation was highest between BC and the South Cascades , and intermediate between BC and the North Cascades .
	manualset3
84017	4	397886	14	13	NULL	0	NULL	BC	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic differentiation was highest between BC and the South Cascades , and intermediate between BC and the North Cascades .
	manualset3
84018	5	397886	14	13	NULL	0	NULL	North Cascades	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic differentiation was highest between BC and the South Cascades , and intermediate between BC and the North Cascades .
	manualset3
84019	1	397887	14	13	NULL	0	NULL	Genetic diversity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic diversity and population structure of Salvia miltiorrhiza Bge in China revealed by ISSR and SRAP .
	manualset3
84021	3	397887	14	13	NULL	0	NULL	Salvia miltiorrhiza Bge	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic diversity and population structure of Salvia miltiorrhiza Bge in China revealed by ISSR and SRAP .
	manualset3
84022	4	397887	14	13	NULL	0	NULL	China	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic diversity and population structure of Salvia miltiorrhiza Bge in China revealed by ISSR and SRAP .
	manualset3
84023	5	397887	14	13	NULL	NULL	NULL	ISSR	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic diversity and population structure of Salvia miltiorrhiza Bge in China revealed by ISSR and SRAP .
	manualset3
84024	6	397887	14	13	NULL	0	NULL	SRAP	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic diversity and population structure of Salvia miltiorrhiza Bge in China revealed by ISSR and SRAP .
	manualset3
84025	1	397888	14	13	NULL	0	NULL	Genetic information	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic information and the life-span of laboratory animal models .
	manualset3
84026	2	397888	14	13	NULL	NULL	NULL	life-span	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic information and the life-span of laboratory animal models .
	manualset3
84027	3	397888	14	13	NULL	0	NULL	 laboratory animal models	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic information and the life-span of laboratory animal models .
	manualset3
84028	1	397889	14	13	NULL	0	NULL	Genetic inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic inhibition of NAD ( P ) H oxidase or administration of uric acid ( a peroxynitrite scavenger ) or N ( G ) - nitro-l-arginine methyl ester ( nonselective NO synthase inhibitor ) significantly attenuated Ang II-induced PA700 nitration , 26S proteasome activation , and reduction of GTP cyclohydrolase I and BH4 .
	manualset3
84029	2	397889	14	13	NULL	0	NULL	NAD ( P ) H oxidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic inhibition of NAD ( P ) H oxidase or administration of uric acid ( a peroxynitrite scavenger ) or N ( G ) - nitro-l-arginine methyl ester ( nonselective NO synthase inhibitor ) significantly attenuated Ang II-induced PA700 nitration , 26S proteasome activation , and reduction of GTP cyclohydrolase I and BH4 .
	manualset3
84030	3	397889	14	13	NULL	0	NULL	administration	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic inhibition of NAD ( P ) H oxidase or administration of uric acid ( a peroxynitrite scavenger ) or N ( G ) - nitro-l-arginine methyl ester ( nonselective NO synthase inhibitor ) significantly attenuated Ang II-induced PA700 nitration , 26S proteasome activation , and reduction of GTP cyclohydrolase I and BH4 .
	manualset3
84031	4	397889	14	13	NULL	0	NULL	uric acid ( a peroxynitrite scavenger ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic inhibition of NAD ( P ) H oxidase or administration of uric acid ( a peroxynitrite scavenger ) or N ( G ) - nitro-l-arginine methyl ester ( nonselective NO synthase inhibitor ) significantly attenuated Ang II-induced PA700 nitration , 26S proteasome activation , and reduction of GTP cyclohydrolase I and BH4 .
	manualset3
84032	5	397889	14	13	NULL	0	NULL	N ( G ) - nitro-l-arginine methyl ester ( nonselective NO synthase inhibitor )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic inhibition of NAD ( P ) H oxidase or administration of uric acid ( a peroxynitrite scavenger ) or N ( G ) - nitro-l-arginine methyl ester ( nonselective NO synthase inhibitor ) significantly attenuated Ang II-induced PA700 nitration , 26S proteasome activation , and reduction of GTP cyclohydrolase I and BH4 .
	manualset3
84035	6	397889	14	13	NULL	NULL	NULL	Ang II-induced PA700 nitration	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic inhibition of NAD ( P ) H oxidase or administration of uric acid ( a peroxynitrite scavenger ) or N ( G ) - nitro-l-arginine methyl ester ( nonselective NO synthase inhibitor ) significantly attenuated Ang II-induced PA700 nitration , 26S proteasome activation , and reduction of GTP cyclohydrolase I and BH4 .
	manualset3
84036	7	397889	14	13	NULL	NULL	NULL	26S proteasome activation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic inhibition of NAD ( P ) H oxidase or administration of uric acid ( a peroxynitrite scavenger ) or N ( G ) - nitro-l-arginine methyl ester ( nonselective NO synthase inhibitor ) significantly attenuated Ang II-induced PA700 nitration , 26S proteasome activation , and reduction of GTP cyclohydrolase I and BH4 .
	manualset3
84039	8	397889	14	13	NULL	NULL	NULL	reduction of GTP cyclohydrolase I and BH4	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic inhibition of NAD ( P ) H oxidase or administration of uric acid ( a peroxynitrite scavenger ) or N ( G ) - nitro-l-arginine methyl ester ( nonselective NO synthase inhibitor ) significantly attenuated Ang II-induced PA700 nitration , 26S proteasome activation , and reduction of GTP cyclohydrolase I and BH4 .
	manualset3
84041	1	397890	14	13	NULL	0	NULL	Genetic instability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic instability and p53 mutations in metastatic foci of mouse urinary bladder carcinomas induced by N-butyl-N - ( 4-hydroxybutyl ) nitrosamine .
	manualset3
84042	2	397890	14	13	NULL	NULL	NULL	p53 mutations	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic instability and p53 mutations in metastatic foci of mouse urinary bladder carcinomas induced by N-butyl-N - ( 4-hydroxybutyl ) nitrosamine .
	manualset3
84044	4	397890	14	13	NULL	0	NULL	metastatic foci	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic instability and p53 mutations in metastatic foci of mouse urinary bladder carcinomas induced by N-butyl-N - ( 4-hydroxybutyl ) nitrosamine .
	manualset3
84045	5	397890	14	13	NULL	0	NULL	mouse	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic instability and p53 mutations in metastatic foci of mouse urinary bladder carcinomas induced by N-butyl-N - ( 4-hydroxybutyl ) nitrosamine .
	manualset3
84046	6	397890	14	13	NULL	0	NULL	urinary bladder carcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic instability and p53 mutations in metastatic foci of mouse urinary bladder carcinomas induced by N-butyl-N - ( 4-hydroxybutyl ) nitrosamine .
	manualset3
84047	7	397890	14	13	NULL	0	NULL	N-butyl-N - ( 4-hydroxybutyl ) nitrosamine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic instability and p53 mutations in metastatic foci of mouse urinary bladder carcinomas induced by N-butyl-N - ( 4-hydroxybutyl ) nitrosamine .
	manualset3
84048	1	397891	14	13	NULL	0	NULL	Genetic instability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic instability of microsatellite sequences in non-small cell lung cancers .
	manualset3
84049	2	397891	14	13	NULL	0	NULL	microsatellite sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic instability of microsatellite sequences in non-small cell lung cancers .
	manualset3
84050	3	397891	14	13	NULL	0	NULL	non-small cell lung cancers	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic instability of microsatellite sequences in non-small cell lung cancers .
	manualset3
84051	1	397892	14	13	NULL	NULL	NULL	Genetic interactions 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic interactions in the - adrenoceptor/G-protein signal transduction pathway and survival after coronary artery bypass grafting : a pilot study .
	manualset3
84052	2	397892	14	13	NULL	0	NULL	adrenoceptor/G-protein signal transduction pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic interactions in the - adrenoceptor/G-protein signal transduction pathway and survival after coronary artery bypass grafting : a pilot study .
	manualset3
84053	3	397892	14	13	NULL	NULL	NULL	survival	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic interactions in the - adrenoceptor/G-protein signal transduction pathway and survival after coronary artery bypass grafting : a pilot study .
	manualset3
84054	4	397892	14	13	NULL	0	NULL	coronary artery bypass grafting 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic interactions in the - adrenoceptor/G-protein signal transduction pathway and survival after coronary artery bypass grafting : a pilot study .
	manualset3
84055	5	397892	14	13	NULL	0	NULL	pilot study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic interactions in the - adrenoceptor/G-protein signal transduction pathway and survival after coronary artery bypass grafting : a pilot study .
	manualset3
84056	1	397893	14	13	NULL	NULL	NULL	Genetic polymorphims	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic polymorphims in promoter region of osteopontin gene may be a marker reflecting hepatitis activity in chronic hepatitis C patients .
	manualset3
84057	2	397893	14	13	NULL	0	NULL	promoter region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic polymorphims in promoter region of osteopontin gene may be a marker reflecting hepatitis activity in chronic hepatitis C patients .
	manualset3
84058	3	397893	14	13	NULL	0	NULL	osteopontin gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic polymorphims in promoter region of osteopontin gene may be a marker reflecting hepatitis activity in chronic hepatitis C patients .
	manualset3
84059	4	397893	14	13	NULL	NULL	NULL	hepatitis activity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic polymorphims in promoter region of osteopontin gene may be a marker reflecting hepatitis activity in chronic hepatitis C patients .
	manualset3
84060	5	397893	14	13	NULL	0	NULL	chronic hepatitis C	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic polymorphims in promoter region of osteopontin gene may be a marker reflecting hepatitis activity in chronic hepatitis C patients .
	manualset3
84061	6	397893	14	13	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic polymorphims in promoter region of osteopontin gene may be a marker reflecting hepatitis activity in chronic hepatitis C patients .
	manualset3
84062	1	397894	14	13	NULL	NULL	NULL	Genetic predisposition	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic predisposition to breast cancer : past , present , and future .
	manualset3
84063	2	397894	14	13	NULL	0	NULL	breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic predisposition to breast cancer : past , present , and future .
	manualset3
84064	3	397894	14	13	NULL	0	NULL	past 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic predisposition to breast cancer : past , present , and future .
	manualset3
84065	4	397894	14	13	NULL	0	NULL	present	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic predisposition to breast cancer : past , present , and future .
	manualset3
84066	5	397894	14	13	NULL	0	NULL	future	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic predisposition to breast cancer : past , present , and future .
	manualset3
84067	1	397895	14	13	NULL	0	NULL	Genetic restriction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic restriction of HIV-1 pathogenesis to AIDS by promoter alleles of IL10 .
	manualset3
84069	3	397895	14	13	NULL	NULL	NULL	HIV-1 pathogenesis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic restriction of HIV-1 pathogenesis to AIDS by promoter alleles of IL10 .
	manualset3
84070	4	397895	14	13	NULL	0	NULL	AIDS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic restriction of HIV-1 pathogenesis to AIDS by promoter alleles of IL10 .
	manualset3
84071	5	397895	14	13	NULL	0	NULL	promoter alleles of IL10	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic restriction of HIV-1 pathogenesis to AIDS by promoter alleles of IL10 .
	manualset3
84072	1	397896	14	13	NULL	0	NULL	Genetic studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic studies on MTP mitogenicity revealed that 90 % of responder DBA/2J X nonresponder C3H/HeJ F1 hybrids had intermediate mitogenic activity .
	manualset3
84073	2	397896	14	13	NULL	NULL	NULL	MTP mitogenicity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic studies on MTP mitogenicity revealed that 90 % of responder DBA/2J X nonresponder C3H/HeJ F1 hybrids had intermediate mitogenic activity .
	manualset3
84074	4	397896	14	13	NULL	NULL	NULL	90 %	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic studies on MTP mitogenicity revealed that 90 % of responder DBA/2J X nonresponder C3H/HeJ F1 hybrids had intermediate mitogenic activity .
	manualset3
84075	5	397896	14	13	NULL	NULL	NULL	responder DBA/2J X nonresponder C3H/HeJ F1 hybrids	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic studies on MTP mitogenicity revealed that 90 % of responder DBA/2J X nonresponder C3H/HeJ F1 hybrids had intermediate mitogenic activity .
	manualset3
84077	6	397896	14	13	NULL	NULL	NULL	mitogenic activity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic studies on MTP mitogenicity revealed that 90 % of responder DBA/2J X nonresponder C3H/HeJ F1 hybrids had intermediate mitogenic activity .
	manualset3
84079	1	397897	14	13	NULL	0	NULL	Genetic variation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic variation in phosphorus ( P ) efficiency exists among wheat ( Triticum aestivum ) and barley ( Hordeum vulgare ) genotypes , but the underlying mechanisms for the variation remain elusive .
	manualset3
84080	1	397897	14	13	NULL	NULL	NULL	phosphorus ( P ) efficiency	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic variation in phosphorus ( P ) efficiency exists among wheat ( Triticum aestivum ) and barley ( Hordeum vulgare ) genotypes , but the underlying mechanisms for the variation remain elusive .
	manualset3
84081	3	397897	14	13	NULL	0	NULL	wheat ( Triticum aestivum ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic variation in phosphorus ( P ) efficiency exists among wheat ( Triticum aestivum ) and barley ( Hordeum vulgare ) genotypes , but the underlying mechanisms for the variation remain elusive .
	manualset3
84082	4	397897	14	13	NULL	0	NULL	barley ( Hordeum vulgare ) genotypes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic variation in phosphorus ( P ) efficiency exists among wheat ( Triticum aestivum ) and barley ( Hordeum vulgare ) genotypes , but the underlying mechanisms for the variation remain elusive .
	manualset3
84083	5	397897	14	13	NULL	NULL	NULL	underlying mechanisms for the variation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic variation in phosphorus ( P ) efficiency exists among wheat ( Triticum aestivum ) and barley ( Hordeum vulgare ) genotypes , but the underlying mechanisms for the variation remain elusive .
	manualset3
84084	1	397898	14	13	NULL	0	NULL	Genetic variation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic variation in the promoter of the lactase gene ( LCT ) is known to be associated with lactase production and is therefore a genetic determinant for either lactase deficiency or lactase persistence during adulthood .
	manualset3
84085	2	397898	14	13	NULL	0	NULL	 promoter of the lactase gene ( LCT )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic variation in the promoter of the lactase gene ( LCT ) is known to be associated with lactase production and is therefore a genetic determinant for either lactase deficiency or lactase persistence during adulthood .
	manualset3
84086	3	397898	14	13	NULL	0	NULL	lactase production 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic variation in the promoter of the lactase gene ( LCT ) is known to be associated with lactase production and is therefore a genetic determinant for either lactase deficiency or lactase persistence during adulthood .
	manualset3
84087	4	397898	14	13	NULL	0	NULL	lactase deficiency	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic variation in the promoter of the lactase gene ( LCT ) is known to be associated with lactase production and is therefore a genetic determinant for either lactase deficiency or lactase persistence during adulthood .
	manualset3
84088	5	397898	14	13	NULL	0	NULL	lactase persistence 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic variation in the promoter of the lactase gene ( LCT ) is known to be associated with lactase production and is therefore a genetic determinant for either lactase deficiency or lactase persistence during adulthood .
	manualset3
84100	6	397898	14	13	NULL	NULL	NULL	adulthood	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic variation in the promoter of the lactase gene ( LCT ) is known to be associated with lactase production and is therefore a genetic determinant for either lactase deficiency or lactase persistence during adulthood .
	manualset3
84101	7	397898	14	13	NULL	NULL	NULL	genetic determinant 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic variation in the promoter of the lactase gene ( LCT ) is known to be associated with lactase production and is therefore a genetic determinant for either lactase deficiency or lactase persistence during adulthood .
	manualset3
84090	1	397899	14	13	NULL	NULL	NULL	Genetics of Parthenogenesis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetics of Parthenogenesis in DROSOPHILA MELANOGASTER .
	manualset3
84091	2	397899	14	13	NULL	NULL	NULL	DROSOPHILA MELANOGASTER 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetics of Parthenogenesis in DROSOPHILA MELANOGASTER .
	manualset3
84092	1	397900	14	13	NULL	NULL	NULL	Genetics	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetics of aryl hydrocarbon hydroxylase induction in mice : additive inheritance in crosses between C3H-HeJ and DBA-2J .
	manualset3
84093	2	397900	14	13	NULL	NULL	NULL	aryl hydrocarbon hydroxylase	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetics of aryl hydrocarbon hydroxylase induction in mice : additive inheritance in crosses between C3H-HeJ and DBA-2J .
	manualset3
84094	3	397900	14	13	NULL	NULL	NULL	induction	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetics of aryl hydrocarbon hydroxylase induction in mice : additive inheritance in crosses between C3H-HeJ and DBA-2J .
	manualset3
84095	4	397900	14	13	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetics of aryl hydrocarbon hydroxylase induction in mice : additive inheritance in crosses between C3H-HeJ and DBA-2J .
	manualset3
84096	5	397900	14	13	NULL	0	NULL	additive inheritance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetics of aryl hydrocarbon hydroxylase induction in mice : additive inheritance in crosses between C3H-HeJ and DBA-2J .
	manualset3
84097	6	397900	14	13	NULL	0	NULL	crosses 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetics of aryl hydrocarbon hydroxylase induction in mice : additive inheritance in crosses between C3H-HeJ and DBA-2J .
	manualset3
84098	7	397900	14	13	NULL	0	NULL	C3H-HeJ	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetics of aryl hydrocarbon hydroxylase induction in mice : additive inheritance in crosses between C3H-HeJ and DBA-2J .
	manualset3
84099	8	397900	14	13	NULL	0	NULL	 DBA-2J	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetics of aryl hydrocarbon hydroxylase induction in mice : additive inheritance in crosses between C3H-HeJ and DBA-2J .
	manualset3
84102	1	397901	14	13	NULL	0	NULL	Sinonasal mucosal melanoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Sinonasal mucosal melanoma ) .
	manualset3
84103	1	397902	14	13	NULL	NULL	NULL	Genistein	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genistein and C3 transferase toxin did not elevate the cellular cAMP levels .
	manualset3
84104	2	397902	14	13	NULL	0	NULL	C3 transferase toxin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Genistein and C3 transferase toxin did not elevate the cellular cAMP levels .
	manualset3
84105	3	397902	14	13	NULL	NULL	NULL	cellular cAMP 	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genistein and C3 transferase toxin did not elevate the cellular cAMP levels .
	manualset3
84114	4	397902	14	13	NULL	0	NULL	 levels 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Genistein and C3 transferase toxin did not elevate the cellular cAMP levels .
	manualset3
84107	1	397903	14	13	NULL	0	NULL	Genistein	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Genistein induced significant increases in the number of FSH cells ( by 21 % ) and LH cells ( by 20 % ) per mm ( 2 ) compared to corresponding controls .
	manualset3
84108	2	397903	14	13	NULL	0	NULL	FSH cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Genistein induced significant increases in the number of FSH cells ( by 21 % ) and LH cells ( by 20 % ) per mm ( 2 ) compared to corresponding controls .
	manualset3
84109	3	397903	14	13	NULL	NULL	NULL	by 21% per mm (2)	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genistein induced significant increases in the number of FSH cells ( by 21 % ) and LH cells ( by 20 % ) per mm ( 2 ) compared to corresponding controls .
	manualset3
84110	4	397903	14	13	NULL	NULL	NULL	LH cells 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genistein induced significant increases in the number of FSH cells ( by 21 % ) and LH cells ( by 20 % ) per mm ( 2 ) compared to corresponding controls .
	manualset3
84111	5	397903	14	13	NULL	NULL	NULL	by 20% per mm (2)	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genistein induced significant increases in the number of FSH cells ( by 21 % ) and LH cells ( by 20 % ) per mm ( 2 ) compared to corresponding controls .
	manualset3
84113	6	397903	14	13	NULL	NULL	NULL	corresponding controls	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genistein induced significant increases in the number of FSH cells ( by 21 % ) and LH cells ( by 20 % ) per mm ( 2 ) compared to corresponding controls .
	manualset3
84115	1	397904	14	13	NULL	0	NULL	Genome-wide association studies ( GWAS )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genome-wide association studies ( GWAS ) have led to the identification of more than 100 common , low-penetrance loci for cancer .
	manualset3
84116	2	397904	14	13	NULL	NULL	NULL	identification	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genome-wide association studies ( GWAS ) have led to the identification of more than 100 common , low-penetrance loci for cancer .
	manualset3
84117	3	397904	14	13	NULL	0	NULL	more than 100 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genome-wide association studies ( GWAS ) have led to the identification of more than 100 common , low-penetrance loci for cancer .
	manualset3
84118	4	397904	14	13	NULL	NULL	NULL	low-penetrance loci	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genome-wide association studies ( GWAS ) have led to the identification of more than 100 common , low-penetrance loci for cancer .
	manualset3
84119	5	397904	14	13	NULL	0	NULL	cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Genome-wide association studies ( GWAS ) have led to the identification of more than 100 common , low-penetrance loci for cancer .
	manualset3
84120	1	397905	14	13	NULL	0	NULL	Genome-wide association study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genome-wide association study of PR interval .
	manualset3
84121	2	397905	14	13	NULL	NULL	NULL	PR interval	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genome-wide association study of PR interval .
	manualset3
84134	1	397907	14	13	NULL	0	NULL	Genomic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genomic analysis of the major bovine milk protein genes .
	manualset3
84135	2	397907	14	13	NULL	0	NULL	bovine	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Genomic analysis of the major bovine milk protein genes .
	manualset3
84136	3	397907	14	13	NULL	0	NULL	milk protein genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Genomic analysis of the major bovine milk protein genes .
	manualset3
84143	1	397909	14	13	NULL	0	NULL	Genomic maps	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Genomic maps of long noncoding RNA occupancy reveal principles of RNA-chromatin interactions .
	manualset3
84144	2	397909	14	13	NULL	NULL	NULL	long noncoding RNA occupancy	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genomic maps of long noncoding RNA occupancy reveal principles of RNA-chromatin interactions .
	manualset3
84145	3	397909	14	13	NULL	NULL	NULL	principles of RNA-chromatin interactions	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genomic maps of long noncoding RNA occupancy reveal principles of RNA-chromatin interactions .
	manualset3
84146	1	397910	14	13	NULL	NULL	NULL	Airflowmeter	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Airflowmeter -- a simple apparatus for lung function tests ) .
	manualset3
84147	2	397910	14	13	NULL	0	NULL	lung function tests	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Airflowmeter -- a simple apparatus for lung function tests ) .
	manualset3
84148	1	397911	14	13	NULL	0	NULL	Situation-simulating games	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Situation-simulating games in the teaching of obstetrics ) .
	manualset3
84209	2	397911	14	13	NULL	0	NULL	teaching 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Situation-simulating games in the teaching of obstetrics ) .
	manualset3
84210	3	397911	14	13	NULL	NULL	NULL	obstetrics 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Situation-simulating games in the teaching of obstetrics ) .
	manualset3
84149	1	397912	14	13	NULL	NULL	NULL	Genomic profiling 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genomic profiling of peripheral T-cell lymphoma , unspecified , and anaplastic large T-cell lymphoma delineates novel recurrent chromosomal alterations .
	manualset3
84150	2	397912	14	13	NULL	NULL	NULL	peripheral T-cell lymphoma 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genomic profiling of peripheral T-cell lymphoma , unspecified , and anaplastic large T-cell lymphoma delineates novel recurrent chromosomal alterations .
	manualset3
84151	3	397912	14	13	NULL	0	NULL	anaplastic large T-cell lymphoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Genomic profiling of peripheral T-cell lymphoma , unspecified , and anaplastic large T-cell lymphoma delineates novel recurrent chromosomal alterations .
	manualset3
84152	4	397912	14	13	NULL	0	NULL	novel recurrent chromosomal alterations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Genomic profiling of peripheral T-cell lymphoma , unspecified , and anaplastic large T-cell lymphoma delineates novel recurrent chromosomal alterations .
	manualset3
84153	1	397913	14	13	NULL	0	NULL	Genomic profiling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genomic profiling of plasmablastic lymphoma using array comparative genomic hybridization ( aCGH ) : revealing significant overlapping genomic lesions with diffuse large B-cell lymphoma .
	manualset3
84154	2	397913	14	13	NULL	0	NULL	plasmablastic lymphoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Genomic profiling of plasmablastic lymphoma using array comparative genomic hybridization ( aCGH ) : revealing significant overlapping genomic lesions with diffuse large B-cell lymphoma .
	manualset3
84155	3	397913	14	13	NULL	0	NULL	 array comparative genomic hybridization ( aCGH ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genomic profiling of plasmablastic lymphoma using array comparative genomic hybridization ( aCGH ) : revealing significant overlapping genomic lesions with diffuse large B-cell lymphoma .
	manualset3
84156	4	397913	14	13	NULL	0	NULL	overlapping genomic lesions	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Genomic profiling of plasmablastic lymphoma using array comparative genomic hybridization ( aCGH ) : revealing significant overlapping genomic lesions with diffuse large B-cell lymphoma .
	manualset3
84157	5	397913	14	13	NULL	0	NULL	diffuse large B-cell lymphoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Genomic profiling of plasmablastic lymphoma using array comparative genomic hybridization ( aCGH ) : revealing significant overlapping genomic lesions with diffuse large B-cell lymphoma .
	manualset3
84158	1	397914	14	13	NULL	NULL	NULL	Genoprotective properties	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genoprotective properties in BTK-8L correlate to some extent with the lowering of the death rate of experimental animals at the early stage of intoxication by chlorofos at the prophylactic injection of the preparation , which , nevertheless , was not so significant , as in the case of intoxication by tetrachloromethane .
	manualset3
84159	2	397914	14	13	NULL	0	NULL	BTK-8L	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Genoprotective properties in BTK-8L correlate to some extent with the lowering of the death rate of experimental animals at the early stage of intoxication by chlorofos at the prophylactic injection of the preparation , which , nevertheless , was not so significant , as in the case of intoxication by tetrachloromethane .
	manualset3
84160	3	397914	14	13	NULL	NULL	NULL	lowering of the death rate	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genoprotective properties in BTK-8L correlate to some extent with the lowering of the death rate of experimental animals at the early stage of intoxication by chlorofos at the prophylactic injection of the preparation , which , nevertheless , was not so significant , as in the case of intoxication by tetrachloromethane .
	manualset3
84161	4	397914	14	13	NULL	0	NULL	experimental animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Genoprotective properties in BTK-8L correlate to some extent with the lowering of the death rate of experimental animals at the early stage of intoxication by chlorofos at the prophylactic injection of the preparation , which , nevertheless , was not so significant , as in the case of intoxication by tetrachloromethane .
	manualset3
84162	5	397914	14	13	NULL	0	NULL	early stage of intoxication	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Genoprotective properties in BTK-8L correlate to some extent with the lowering of the death rate of experimental animals at the early stage of intoxication by chlorofos at the prophylactic injection of the preparation , which , nevertheless , was not so significant , as in the case of intoxication by tetrachloromethane .
	manualset3
84163	6	397914	14	13	NULL	0	NULL	chlorofos 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Genoprotective properties in BTK-8L correlate to some extent with the lowering of the death rate of experimental animals at the early stage of intoxication by chlorofos at the prophylactic injection of the preparation , which , nevertheless , was not so significant , as in the case of intoxication by tetrachloromethane .
	manualset3
84164	7	397914	14	13	NULL	0	NULL	prophylactic injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Genoprotective properties in BTK-8L correlate to some extent with the lowering of the death rate of experimental animals at the early stage of intoxication by chlorofos at the prophylactic injection of the preparation , which , nevertheless , was not so significant , as in the case of intoxication by tetrachloromethane .
	manualset3
84165	8	397914	14	13	NULL	NULL	NULL	intoxication 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genoprotective properties in BTK-8L correlate to some extent with the lowering of the death rate of experimental animals at the early stage of intoxication by chlorofos at the prophylactic injection of the preparation , which , nevertheless , was not so significant , as in the case of intoxication by tetrachloromethane .
	manualset3
84166	9	397914	14	13	NULL	0	NULL	tetrachloromethane	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Genoprotective properties in BTK-8L correlate to some extent with the lowering of the death rate of experimental animals at the early stage of intoxication by chlorofos at the prophylactic injection of the preparation , which , nevertheless , was not so significant , as in the case of intoxication by tetrachloromethane .
	manualset3
84167	1	397915	14	13	NULL	0	NULL	Genotypes	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Genotypes of the two loci were identified by direct sequencing , and for site 85 of the mtLSU locus , three allele-specific PCR assays were used .
	manualset3
84168	2	397915	14	13	NULL	NULL	NULL	two	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genotypes of the two loci were identified by direct sequencing , and for site 85 of the mtLSU locus , three allele-specific PCR assays were used .
	manualset3
84169	3	397915	14	13	NULL	0	NULL	loci	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Genotypes of the two loci were identified by direct sequencing , and for site 85 of the mtLSU locus , three allele-specific PCR assays were used .
	manualset3
84170	4	397915	14	13	NULL	0	NULL	direct sequencing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genotypes of the two loci were identified by direct sequencing , and for site 85 of the mtLSU locus , three allele-specific PCR assays were used .
	manualset3
84171	5	397915	14	13	NULL	NULL	NULL	site 85 of the mtLSU locus 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genotypes of the two loci were identified by direct sequencing , and for site 85 of the mtLSU locus , three allele-specific PCR assays were used .
	manualset3
84173	6	397915	14	13	NULL	NULL	NULL	three	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genotypes of the two loci were identified by direct sequencing , and for site 85 of the mtLSU locus , three allele-specific PCR assays were used .
	manualset3
84174	7	397915	14	13	NULL	NULL	NULL	allele-specific PCR assays 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genotypes of the two loci were identified by direct sequencing , and for site 85 of the mtLSU locus , three allele-specific PCR assays were used .
	manualset3
84175	1	397916	14	13	NULL	0	NULL	Genotypic and phenotypic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genotypic and phenotypic analysis of Mycoplasma fermentans strains isolated from different host tissues .
	manualset3
84176	2	397916	14	13	NULL	NULL	NULL	Mycoplasma fermentans strains	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genotypic and phenotypic analysis of Mycoplasma fermentans strains isolated from different host tissues .
	manualset3
84177	3	397916	14	13	NULL	0	NULL	different host tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Genotypic and phenotypic analysis of Mycoplasma fermentans strains isolated from different host tissues .
	manualset3
84178	1	397917	14	13	NULL	0	NULL	Genotypic and phenotypic stability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Genotypic and phenotypic stability of Helicobacter pylori markers in a nine-year follow-up study of patients with noneradicated infection .
	manualset3
84179	2	397917	14	13	NULL	0	NULL	Helicobacter pylori markers 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Genotypic and phenotypic stability of Helicobacter pylori markers in a nine-year follow-up study of patients with noneradicated infection .
	manualset3
84180	3	397917	14	13	NULL	0	NULL	nine-year	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Genotypic and phenotypic stability of Helicobacter pylori markers in a nine-year follow-up study of patients with noneradicated infection .
	manualset3
84181	4	397917	14	13	NULL	0	NULL	follow-up study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genotypic and phenotypic stability of Helicobacter pylori markers in a nine-year follow-up study of patients with noneradicated infection .
	manualset3
84182	5	397917	14	13	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Genotypic and phenotypic stability of Helicobacter pylori markers in a nine-year follow-up study of patients with noneradicated infection .
	manualset3
84183	6	397917	14	13	NULL	0	NULL	noneradicated infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Genotypic and phenotypic stability of Helicobacter pylori markers in a nine-year follow-up study of patients with noneradicated infection .
	manualset3
84184	1	397918	14	13	NULL	0	NULL	Genotyping or phenotyping 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genotyping or phenotyping needs to be introduced in clinical laboratories .
	manualset3
84185	2	397918	14	13	NULL	NULL	NULL	clinical laboratories	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genotyping or phenotyping needs to be introduced in clinical laboratories .
	manualset3
84186	1	397919	14	13	NULL	0	NULL	Gentamicin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Gentamicin ( 2.5 microgram/ml ) , kanamycin ( 31.2 microgram/ml ) , neomycin ( 62.5 microgram/ml ) , and tobramycin ( 2.5 microgram/ml ) were the only antibacterials tested which controlled microbial growth without affecting sperm viability for up to 24 hr storage at 5 C. Tobramycin maintained fertility equal to that of the non-antibiotic control up to 24 hr storage .
	manualset3
84187	2	397919	14	13	NULL	0	NULL	2.5 microgram/ml	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Gentamicin ( 2.5 microgram/ml ) , kanamycin ( 31.2 microgram/ml ) , neomycin ( 62.5 microgram/ml ) , and tobramycin ( 2.5 microgram/ml ) were the only antibacterials tested which controlled microbial growth without affecting sperm viability for up to 24 hr storage at 5 C. Tobramycin maintained fertility equal to that of the non-antibiotic control up to 24 hr storage .
	manualset3
84188	3	397919	14	13	NULL	0	NULL	kanamycin 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Gentamicin ( 2.5 microgram/ml ) , kanamycin ( 31.2 microgram/ml ) , neomycin ( 62.5 microgram/ml ) , and tobramycin ( 2.5 microgram/ml ) were the only antibacterials tested which controlled microbial growth without affecting sperm viability for up to 24 hr storage at 5 C. Tobramycin maintained fertility equal to that of the non-antibiotic control up to 24 hr storage .
	manualset3
84189	4	397919	14	13	NULL	0	NULL	 31.2 microgram/ml	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Gentamicin ( 2.5 microgram/ml ) , kanamycin ( 31.2 microgram/ml ) , neomycin ( 62.5 microgram/ml ) , and tobramycin ( 2.5 microgram/ml ) were the only antibacterials tested which controlled microbial growth without affecting sperm viability for up to 24 hr storage at 5 C. Tobramycin maintained fertility equal to that of the non-antibiotic control up to 24 hr storage .
	manualset3
84190	5	397919	14	13	NULL	0	NULL	 neomycin 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Gentamicin ( 2.5 microgram/ml ) , kanamycin ( 31.2 microgram/ml ) , neomycin ( 62.5 microgram/ml ) , and tobramycin ( 2.5 microgram/ml ) were the only antibacterials tested which controlled microbial growth without affecting sperm viability for up to 24 hr storage at 5 C. Tobramycin maintained fertility equal to that of the non-antibiotic control up to 24 hr storage .
	manualset3
84191	6	397919	14	13	NULL	NULL	NULL	62.5 microgram/ml 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gentamicin ( 2.5 microgram/ml ) , kanamycin ( 31.2 microgram/ml ) , neomycin ( 62.5 microgram/ml ) , and tobramycin ( 2.5 microgram/ml ) were the only antibacterials tested which controlled microbial growth without affecting sperm viability for up to 24 hr storage at 5 C. Tobramycin maintained fertility equal to that of the non-antibiotic control up to 24 hr storage .
	manualset3
84192	7	397919	14	13	NULL	0	NULL	tobramycin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Gentamicin ( 2.5 microgram/ml ) , kanamycin ( 31.2 microgram/ml ) , neomycin ( 62.5 microgram/ml ) , and tobramycin ( 2.5 microgram/ml ) were the only antibacterials tested which controlled microbial growth without affecting sperm viability for up to 24 hr storage at 5 C. Tobramycin maintained fertility equal to that of the non-antibiotic control up to 24 hr storage .
	manualset3
84193	8	397919	14	13	NULL	0	NULL	2.5 microgram/ml 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Gentamicin ( 2.5 microgram/ml ) , kanamycin ( 31.2 microgram/ml ) , neomycin ( 62.5 microgram/ml ) , and tobramycin ( 2.5 microgram/ml ) were the only antibacterials tested which controlled microbial growth without affecting sperm viability for up to 24 hr storage at 5 C. Tobramycin maintained fertility equal to that of the non-antibiotic control up to 24 hr storage .
	manualset3
84194	9	397919	14	13	NULL	0	NULL	antibacterials	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Gentamicin ( 2.5 microgram/ml ) , kanamycin ( 31.2 microgram/ml ) , neomycin ( 62.5 microgram/ml ) , and tobramycin ( 2.5 microgram/ml ) were the only antibacterials tested which controlled microbial growth without affecting sperm viability for up to 24 hr storage at 5 C. Tobramycin maintained fertility equal to that of the non-antibiotic control up to 24 hr storage .
	manualset3
84195	10	397919	14	13	NULL	NULL	NULL	microbial growth	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gentamicin ( 2.5 microgram/ml ) , kanamycin ( 31.2 microgram/ml ) , neomycin ( 62.5 microgram/ml ) , and tobramycin ( 2.5 microgram/ml ) were the only antibacterials tested which controlled microbial growth without affecting sperm viability for up to 24 hr storage at 5 C. Tobramycin maintained fertility equal to that of the non-antibiotic control up to 24 hr storage .
	manualset3
84196	11	397919	14	13	NULL	NULL	NULL	sperm viability	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gentamicin ( 2.5 microgram/ml ) , kanamycin ( 31.2 microgram/ml ) , neomycin ( 62.5 microgram/ml ) , and tobramycin ( 2.5 microgram/ml ) were the only antibacterials tested which controlled microbial growth without affecting sperm viability for up to 24 hr storage at 5 C. Tobramycin maintained fertility equal to that of the non-antibiotic control up to 24 hr storage .
	manualset3
84197	12	397919	14	13	NULL	0	NULL	24 hr	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Gentamicin ( 2.5 microgram/ml ) , kanamycin ( 31.2 microgram/ml ) , neomycin ( 62.5 microgram/ml ) , and tobramycin ( 2.5 microgram/ml ) were the only antibacterials tested which controlled microbial growth without affecting sperm viability for up to 24 hr storage at 5 C. Tobramycin maintained fertility equal to that of the non-antibiotic control up to 24 hr storage .
	manualset3
84198	13	397919	14	13	NULL	0	NULL	5 C	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Gentamicin ( 2.5 microgram/ml ) , kanamycin ( 31.2 microgram/ml ) , neomycin ( 62.5 microgram/ml ) , and tobramycin ( 2.5 microgram/ml ) were the only antibacterials tested which controlled microbial growth without affecting sperm viability for up to 24 hr storage at 5 C. Tobramycin maintained fertility equal to that of the non-antibiotic control up to 24 hr storage .
	manualset3
84199	14	397919	14	13	NULL	0	NULL	Tobramycin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Gentamicin ( 2.5 microgram/ml ) , kanamycin ( 31.2 microgram/ml ) , neomycin ( 62.5 microgram/ml ) , and tobramycin ( 2.5 microgram/ml ) were the only antibacterials tested which controlled microbial growth without affecting sperm viability for up to 24 hr storage at 5 C. Tobramycin maintained fertility equal to that of the non-antibiotic control up to 24 hr storage .
	manualset3
84200	15	397919	14	13	NULL	NULL	NULL	fertility 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gentamicin ( 2.5 microgram/ml ) , kanamycin ( 31.2 microgram/ml ) , neomycin ( 62.5 microgram/ml ) , and tobramycin ( 2.5 microgram/ml ) were the only antibacterials tested which controlled microbial growth without affecting sperm viability for up to 24 hr storage at 5 C. Tobramycin maintained fertility equal to that of the non-antibiotic control up to 24 hr storage .
	manualset3
84201	16	397919	14	13	NULL	NULL	NULL	non-antibiotic control 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gentamicin ( 2.5 microgram/ml ) , kanamycin ( 31.2 microgram/ml ) , neomycin ( 62.5 microgram/ml ) , and tobramycin ( 2.5 microgram/ml ) were the only antibacterials tested which controlled microbial growth without affecting sperm viability for up to 24 hr storage at 5 C. Tobramycin maintained fertility equal to that of the non-antibiotic control up to 24 hr storage .
	manualset3
84202	17	397919	14	13	NULL	0	NULL	24 hr 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Gentamicin ( 2.5 microgram/ml ) , kanamycin ( 31.2 microgram/ml ) , neomycin ( 62.5 microgram/ml ) , and tobramycin ( 2.5 microgram/ml ) were the only antibacterials tested which controlled microbial growth without affecting sperm viability for up to 24 hr storage at 5 C. Tobramycin maintained fertility equal to that of the non-antibiotic control up to 24 hr storage .
	manualset3
84203	1	397920	14	13	NULL	0	NULL	Geobacillus stearothermophilus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Geobacillus stearothermophilus has been used under mesophilic and static cultivation conditions using wool as the main carbon source .
	manualset3
84204	2	397920	14	13	NULL	0	NULL	mesophilic and static cultivation conditions	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Geobacillus stearothermophilus has been used under mesophilic and static cultivation conditions using wool as the main carbon source .
	manualset3
84205	3	397920	14	13	NULL	NULL	NULL	wool	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Geobacillus stearothermophilus has been used under mesophilic and static cultivation conditions using wool as the main carbon source .
	manualset3
84206	4	397920	14	13	NULL	0	NULL	carbon 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Geobacillus stearothermophilus has been used under mesophilic and static cultivation conditions using wool as the main carbon source .
	manualset3
84229	1	397921	14	13	NULL	0	NULL	Slovak 	Language												NULL		0	NULL	NULL	NULL	NULL	NULL	( Slovak verbal audiometry ) .
	manualset3
84230	2	397921	14	13	NULL	0	NULL	verbal audiometry 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	( Slovak verbal audiometry ) .
	manualset3
84231	1	397922	14	13	NULL	0	NULL	George Eliot	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	George Eliot and specific learning disorders .
	manualset3
84232	2	397922	14	13	NULL	0	NULL	specific learning disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	George Eliot and specific learning disorders .
	manualset3
84233	1	397923	14	13	NULL	0	NULL	Gestational diabetes mellitus ( GDM )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Gestational diabetes mellitus ( GDM ) is a risk factor for both Type 2 diabetes ( DM2 ) and insulin-resistance syndrome ( IRS ) .
	manualset3
84234	2	397923	14	13	NULL	0	NULL	risk factor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gestational diabetes mellitus ( GDM ) is a risk factor for both Type 2 diabetes ( DM2 ) and insulin-resistance syndrome ( IRS ) .
	manualset3
84235	3	397923	14	13	NULL	0	NULL	 Type 2 diabetes ( DM2 ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Gestational diabetes mellitus ( GDM ) is a risk factor for both Type 2 diabetes ( DM2 ) and insulin-resistance syndrome ( IRS ) .
	manualset3
84236	4	397923	14	13	NULL	0	NULL	insulin-resistance syndrome ( IRS )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Gestational diabetes mellitus ( GDM ) is a risk factor for both Type 2 diabetes ( DM2 ) and insulin-resistance syndrome ( IRS ) .
	manualset3
84237	1	397924	14	13	NULL	0	NULL	Giant cell arteritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Giant cell arteritis of the uterus and adnexa .
	manualset3
84238	2	397924	14	13	NULL	0	NULL	uterus	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Giant cell arteritis of the uterus and adnexa .
	manualset3
84239	3	397924	14	13	NULL	0	NULL	adnexa	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Giant cell arteritis of the uterus and adnexa .
	manualset3
84240	1	397925	14	13	NULL	0	NULL	Giant cell pneumonia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Giant cell pneumonia is a rare and uncommon type of lung infection developing as a complication of measles , especially in immunocompromised patients , whether their immune systems are affected primarily or whether they have acquired immune defects .
	manualset3
84241	2	397925	14	13	NULL	0	NULL	lung infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Giant cell pneumonia is a rare and uncommon type of lung infection developing as a complication of measles , especially in immunocompromised patients , whether their immune systems are affected primarily or whether they have acquired immune defects .
	manualset3
84242	3	397925	14	13	NULL	NULL	NULL	complication of measles	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Giant cell pneumonia is a rare and uncommon type of lung infection developing as a complication of measles , especially in immunocompromised patients , whether their immune systems are affected primarily or whether they have acquired immune defects .
	manualset3
84243	4	397925	14	13	NULL	0	NULL	 immunocompromised patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Giant cell pneumonia is a rare and uncommon type of lung infection developing as a complication of measles , especially in immunocompromised patients , whether their immune systems are affected primarily or whether they have acquired immune defects .
	manualset3
84244	5	397925	14	13	NULL	NULL	NULL	immune systems	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Giant cell pneumonia is a rare and uncommon type of lung infection developing as a complication of measles , especially in immunocompromised patients , whether their immune systems are affected primarily or whether they have acquired immune defects .
	manualset3
84245	6	397925	14	13	NULL	0	NULL	acquired immune defects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Giant cell pneumonia is a rare and uncommon type of lung infection developing as a complication of measles , especially in immunocompromised patients , whether their immune systems are affected primarily or whether they have acquired immune defects .
	manualset3
84246	1	397926	14	13	NULL	0	NULL	Giardia lamblia	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Giardia lamblia was the most frequent species found .
	manualset3
84248	1	397927	14	13	NULL	0	NULL	Small bridges with inlay and attachment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Small bridges with inlay and attachment : the prosthetic solution for limited tooth gaps ) .
	manualset3
84249	2	397927	14	13	NULL	NULL	NULL	prosthetic solution	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Small bridges with inlay and attachment : the prosthetic solution for limited tooth gaps ) .
	manualset3
84250	3	397927	14	13	NULL	0	NULL	limited tooth gaps	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Small bridges with inlay and attachment : the prosthetic solution for limited tooth gaps ) .
	manualset3
84251	1	397928	14	13	NULL	0	NULL	Gilding the lilly	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Gilding the lilly : comments on the training based model .
	manualset3
84252	2	397928	14	13	NULL	0	NULL	training based model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Gilding the lilly : comments on the training based model .
	manualset3
84253	1	397929	14	13	NULL	0	NULL	Gilts 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Gilts exhibited elevated concentrations of NE in the olfactory bulbs ( OB ) , hypothalamus , pons , and corpus trapezoideum-locus ceruleus ( LC ) compared to lower concentrations in corresponding areas of sows .
	manualset3
84254	2	397929	14	13	NULL	NULL	NULL	elevated concentrations 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gilts exhibited elevated concentrations of NE in the olfactory bulbs ( OB ) , hypothalamus , pons , and corpus trapezoideum-locus ceruleus ( LC ) compared to lower concentrations in corresponding areas of sows .
	manualset3
84255	3	397929	14	13	NULL	0	NULL	NE	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Gilts exhibited elevated concentrations of NE in the olfactory bulbs ( OB ) , hypothalamus , pons , and corpus trapezoideum-locus ceruleus ( LC ) compared to lower concentrations in corresponding areas of sows .
	manualset3
84256	4	397929	14	13	NULL	NULL	NULL	olfactory bulbs ( OB )	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gilts exhibited elevated concentrations of NE in the olfactory bulbs ( OB ) , hypothalamus , pons , and corpus trapezoideum-locus ceruleus ( LC ) compared to lower concentrations in corresponding areas of sows .
	manualset3
84257	5	397929	14	13	NULL	NULL	NULL	hypothalamus	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gilts exhibited elevated concentrations of NE in the olfactory bulbs ( OB ) , hypothalamus , pons , and corpus trapezoideum-locus ceruleus ( LC ) compared to lower concentrations in corresponding areas of sows .
	manualset3
84258	6	397929	14	13	NULL	NULL	NULL	 pons	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gilts exhibited elevated concentrations of NE in the olfactory bulbs ( OB ) , hypothalamus , pons , and corpus trapezoideum-locus ceruleus ( LC ) compared to lower concentrations in corresponding areas of sows .
	manualset3
84259	7	397929	14	13	NULL	NULL	NULL	corpus trapezoideum-locus ceruleus ( LC )	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gilts exhibited elevated concentrations of NE in the olfactory bulbs ( OB ) , hypothalamus , pons , and corpus trapezoideum-locus ceruleus ( LC ) compared to lower concentrations in corresponding areas of sows .
	manualset3
84260	8	397929	14	13	NULL	NULL	NULL	lower concentrations	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gilts exhibited elevated concentrations of NE in the olfactory bulbs ( OB ) , hypothalamus , pons , and corpus trapezoideum-locus ceruleus ( LC ) compared to lower concentrations in corresponding areas of sows .
	manualset3
84261	9	397929	14	13	NULL	NULL	NULL	corresponding areas	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gilts exhibited elevated concentrations of NE in the olfactory bulbs ( OB ) , hypothalamus , pons , and corpus trapezoideum-locus ceruleus ( LC ) compared to lower concentrations in corresponding areas of sows .
	manualset3
84262	10	397929	14	13	NULL	0	NULL	sows	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Gilts exhibited elevated concentrations of NE in the olfactory bulbs ( OB ) , hypothalamus , pons , and corpus trapezoideum-locus ceruleus ( LC ) compared to lower concentrations in corresponding areas of sows .
	manualset3
84263	1	397930	14	13	NULL	0	NULL	Gilts 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Gilts remained on their respective experimental diets and with their penmates throughout the nursery , growing , and finishing phases .
	manualset3
84264	2	397930	14	13	NULL	0	NULL	respective experimental diets 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Gilts remained on their respective experimental diets and with their penmates throughout the nursery , growing , and finishing phases .
	manualset3
84265	3	397930	14	13	NULL	0	NULL	penmates 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Gilts remained on their respective experimental diets and with their penmates throughout the nursery , growing , and finishing phases .
	manualset3
84266	4	397930	14	13	NULL	NULL	NULL	nursery  phase	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gilts remained on their respective experimental diets and with their penmates throughout the nursery , growing , and finishing phases .
	manualset3
84267	5	397930	14	13	NULL	NULL	NULL	growing phase	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gilts remained on their respective experimental diets and with their penmates throughout the nursery , growing , and finishing phases .
	manualset3
84268	6	397930	14	13	NULL	NULL	NULL	finishing phase	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gilts remained on their respective experimental diets and with their penmates throughout the nursery , growing , and finishing phases .
	manualset3
84506	3	397931	14	13	NULL	0	NULL	 increased morbidity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Given a certain severity of crash and of injury , it is unclear whether acute and/or chronic alcohol use leads to increased morbidity , mortality or a more complicated hospital course after motor vehicle collisions .
	manualset3
84507	4	397931	14	13	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Given a certain severity of crash and of injury , it is unclear whether acute and/or chronic alcohol use leads to increased morbidity , mortality or a more complicated hospital course after motor vehicle collisions .
	manualset3
84508	5	397931	14	13	NULL	0	NULL	more complicated hospital course	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Given a certain severity of crash and of injury , it is unclear whether acute and/or chronic alcohol use leads to increased morbidity , mortality or a more complicated hospital course after motor vehicle collisions .
	manualset3
84509	6	397931	14	13	NULL	NULL	NULL	motor vehicle collisions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Given a certain severity of crash and of injury , it is unclear whether acute and/or chronic alcohol use leads to increased morbidity , mortality or a more complicated hospital course after motor vehicle collisions .
	manualset3
84510	7	397931	14	13	NULL	NULL	NULL	certain severity of crash and of injury	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Given a certain severity of crash and of injury , it is unclear whether acute and/or chronic alcohol use leads to increased morbidity , mortality or a more complicated hospital course after motor vehicle collisions .
	manualset3
85426	1	397931	14	13	NULL	NULL	NULL	acute and/or chronic alcohol use	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Given a certain severity of crash and of injury , it is unclear whether acute and/or chronic alcohol use leads to increased morbidity , mortality or a more complicated hospital course after motor vehicle collisions .
	manualset3
84511	1	397932	14	13	NULL	0	NULL	current findings	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Given our current findings , and because a number of risk factors for sporadic AD serve to lower levels of sAPP - in brains of AD patients , inadequate sAPP - levels may be sufficient to polarize APP processing towards the amyloidogenic , A-producing route .
	manualset3
84512	2	397932	14	13	NULL	NULL	NULL	risk factors	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Given our current findings , and because a number of risk factors for sporadic AD serve to lower levels of sAPP - in brains of AD patients , inadequate sAPP - levels may be sufficient to polarize APP processing towards the amyloidogenic , A-producing route .
	manualset3
84513	3	397932	14	13	NULL	NULL	NULL	sporadic AD	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Given our current findings , and because a number of risk factors for sporadic AD serve to lower levels of sAPP - in brains of AD patients , inadequate sAPP - levels may be sufficient to polarize APP processing towards the amyloidogenic , A-producing route .
	manualset3
84514	4	397932	14	13	NULL	NULL	NULL	 levels of sAPP	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Given our current findings , and because a number of risk factors for sporadic AD serve to lower levels of sAPP - in brains of AD patients , inadequate sAPP - levels may be sufficient to polarize APP processing towards the amyloidogenic , A-producing route .
	manualset3
84515	5	397932	14	13	NULL	0	NULL	brains	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Given our current findings , and because a number of risk factors for sporadic AD serve to lower levels of sAPP - in brains of AD patients , inadequate sAPP - levels may be sufficient to polarize APP processing towards the amyloidogenic , A-producing route .
	manualset3
84516	6	397932	14	13	NULL	0	NULL	AD patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Given our current findings , and because a number of risk factors for sporadic AD serve to lower levels of sAPP - in brains of AD patients , inadequate sAPP - levels may be sufficient to polarize APP processing towards the amyloidogenic , A-producing route .
	manualset3
84517	7	397932	14	13	NULL	NULL	NULL	inadequate sAPP - levels	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Given our current findings , and because a number of risk factors for sporadic AD serve to lower levels of sAPP - in brains of AD patients , inadequate sAPP - levels may be sufficient to polarize APP processing towards the amyloidogenic , A-producing route .
	manualset3
84518	8	397932	14	13	NULL	NULL	NULL	APP processing	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Given our current findings , and because a number of risk factors for sporadic AD serve to lower levels of sAPP - in brains of AD patients , inadequate sAPP - levels may be sufficient to polarize APP processing towards the amyloidogenic , A-producing route .
	manualset3
84519	9	397932	14	13	NULL	NULL	NULL	amyloidogenic , A-producing route	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Given our current findings , and because a number of risk factors for sporadic AD serve to lower levels of sAPP - in brains of AD patients , inadequate sAPP - levels may be sufficient to polarize APP processing towards the amyloidogenic , A-producing route .
	manualset3
84521	1	397933	14	13	NULL	0	NULL	species x 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Given species x and y , the ordinal binary character cxy of M is defined by cxy ( s ) = 1 if and only if M ( s , x ) & lt ; M ( s , y ) , for all species s. In this paper we present several results concerning the inference of evolutionary trees or phylogenies from ordinal assertions .
	manualset3
84522	2	397933	14	13	NULL	0	NULL	species y	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Given species x and y , the ordinal binary character cxy of M is defined by cxy ( s ) = 1 if and only if M ( s , x ) & lt ; M ( s , y ) , for all species s. In this paper we present several results concerning the inference of evolutionary trees or phylogenies from ordinal assertions .
	manualset3
84523	3	397933	14	13	NULL	0	NULL	ordinal binary character cxy of M 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Given species x and y , the ordinal binary character cxy of M is defined by cxy ( s ) = 1 if and only if M ( s , x ) & lt ; M ( s , y ) , for all species s. In this paper we present several results concerning the inference of evolutionary trees or phylogenies from ordinal assertions .
	manualset3
84525	5	397933	14	13	NULL	0	NULL	1	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Given species x and y , the ordinal binary character cxy of M is defined by cxy ( s ) = 1 if and only if M ( s , x ) & lt ; M ( s , y ) , for all species s. In this paper we present several results concerning the inference of evolutionary trees or phylogenies from ordinal assertions .
	manualset3
84528	8	397933	14	13	NULL	NULL	NULL	species s	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Given species x and y , the ordinal binary character cxy of M is defined by cxy ( s ) = 1 if and only if M ( s , x ) & lt ; M ( s , y ) , for all species s. In this paper we present several results concerning the inference of evolutionary trees or phylogenies from ordinal assertions .
	manualset3
84529	9	397933	14	13	NULL	0	NULL	paper	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	Given species x and y , the ordinal binary character cxy of M is defined by cxy ( s ) = 1 if and only if M ( s , x ) & lt ; M ( s , y ) , for all species s. In this paper we present several results concerning the inference of evolutionary trees or phylogenies from ordinal assertions .
	manualset3
84531	11	397933	14	13	NULL	NULL	NULL	inference of evolutionary trees 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Given species x and y , the ordinal binary character cxy of M is defined by cxy ( s ) = 1 if and only if M ( s , x ) & lt ; M ( s , y ) , for all species s. In this paper we present several results concerning the inference of evolutionary trees or phylogenies from ordinal assertions .
	manualset3
84532	12	397933	14	13	NULL	NULL	NULL	phylogenies from ordinal assertions	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Given species x and y , the ordinal binary character cxy of M is defined by cxy ( s ) = 1 if and only if M ( s , x ) & lt ; M ( s , y ) , for all species s. In this paper we present several results concerning the inference of evolutionary trees or phylogenies from ordinal assertions .
	manualset3
84533	1	397934	14	13	NULL	0	NULL	PP1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Given that PP1 controls fusion , the SNARE complexes that accumulate in glc7 mutants likely represent trans-SNARE complexes .
	manualset3
84534	2	397934	14	13	NULL	0	NULL	fusion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Given that PP1 controls fusion , the SNARE complexes that accumulate in glc7 mutants likely represent trans-SNARE complexes .
	manualset3
84535	3	397934	14	13	NULL	NULL	NULL	SNARE complexes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Given that PP1 controls fusion , the SNARE complexes that accumulate in glc7 mutants likely represent trans-SNARE complexes .
	manualset3
84536	4	397934	14	13	NULL	0	NULL	glc7 mutants	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Given that PP1 controls fusion , the SNARE complexes that accumulate in glc7 mutants likely represent trans-SNARE complexes .
	manualset3
84537	5	397934	14	13	NULL	NULL	NULL	trans-SNARE complexes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Given that PP1 controls fusion , the SNARE complexes that accumulate in glc7 mutants likely represent trans-SNARE complexes .
	manualset3
84538	1	397935	14	13	NULL	0	NULL	PPAR ligands	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Given that PPAR ligands are currently used in medicine as hypolipidemic drugs with excellent tolerance and limited toxicity , PPARalpha activation might offer a novel and potentially low-toxic approach for the treatment of tumor-associated angiogenesis and cancer .
	manualset3
84539	2	397935	14	13	NULL	NULL	NULL	medicine	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Given that PPAR ligands are currently used in medicine as hypolipidemic drugs with excellent tolerance and limited toxicity , PPARalpha activation might offer a novel and potentially low-toxic approach for the treatment of tumor-associated angiogenesis and cancer .
	manualset3
84540	3	397935	14	13	NULL	NULL	NULL	hypolipidemic drugs	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Given that PPAR ligands are currently used in medicine as hypolipidemic drugs with excellent tolerance and limited toxicity , PPARalpha activation might offer a novel and potentially low-toxic approach for the treatment of tumor-associated angiogenesis and cancer .
	manualset3
84541	4	397935	14	13	NULL	0	NULL	excellent tolerance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Given that PPAR ligands are currently used in medicine as hypolipidemic drugs with excellent tolerance and limited toxicity , PPARalpha activation might offer a novel and potentially low-toxic approach for the treatment of tumor-associated angiogenesis and cancer .
	manualset3
84542	5	397935	14	13	NULL	0	NULL	limited toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Given that PPAR ligands are currently used in medicine as hypolipidemic drugs with excellent tolerance and limited toxicity , PPARalpha activation might offer a novel and potentially low-toxic approach for the treatment of tumor-associated angiogenesis and cancer .
	manualset3
84543	6	397935	14	13	NULL	0	NULL	PPARalpha activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Given that PPAR ligands are currently used in medicine as hypolipidemic drugs with excellent tolerance and limited toxicity , PPARalpha activation might offer a novel and potentially low-toxic approach for the treatment of tumor-associated angiogenesis and cancer .
	manualset3
84544	7	397935	14	13	NULL	0	NULL	novel and potentially low-toxic approach 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Given that PPAR ligands are currently used in medicine as hypolipidemic drugs with excellent tolerance and limited toxicity , PPARalpha activation might offer a novel and potentially low-toxic approach for the treatment of tumor-associated angiogenesis and cancer .
	manualset3
84545	8	397935	14	13	NULL	0	NULL	tumor-associated angiogenesis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Given that PPAR ligands are currently used in medicine as hypolipidemic drugs with excellent tolerance and limited toxicity , PPARalpha activation might offer a novel and potentially low-toxic approach for the treatment of tumor-associated angiogenesis and cancer .
	manualset3
84546	9	397935	14	13	NULL	0	NULL	cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Given that PPAR ligands are currently used in medicine as hypolipidemic drugs with excellent tolerance and limited toxicity , PPARalpha activation might offer a novel and potentially low-toxic approach for the treatment of tumor-associated angiogenesis and cancer .
	manualset3
85427	10	397935	14	13	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Given that PPAR ligands are currently used in medicine as hypolipidemic drugs with excellent tolerance and limited toxicity , PPARalpha activation might offer a novel and potentially low-toxic approach for the treatment of tumor-associated angiogenesis and cancer .
	manualset3
84547	1	397936	14	13	NULL	NULL	NULL	Soft-tissue changes	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Soft-tissue changes in the metacarpal area in chronic polyarthritis ) .
	manualset3
84548	2	397936	14	13	NULL	0	NULL	metacarpal area	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Soft-tissue changes in the metacarpal area in chronic polyarthritis ) .
	manualset3
84549	3	397936	14	13	NULL	0	NULL	chronic polyarthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Soft-tissue changes in the metacarpal area in chronic polyarthritis ) .
	manualset3
84561	1	397938	14	13	NULL	NULL	NULL	kinetics of the peptides	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Given the different kinetics of the peptides , a mathematical model was necessary to analyze the oral glucose tolerance test ( OGTT ) data of insulin , C-peptide , and proinsulin in 55 healthy ( NGT ) , 30 impaired glucose-tolerant ( IGT ) , and 31 type 2 diabetic ( T2DM ) subjects .
	manualset3
84562	2	397938	14	13	NULL	0	NULL	mathematical model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the different kinetics of the peptides , a mathematical model was necessary to analyze the oral glucose tolerance test ( OGTT ) data of insulin , C-peptide , and proinsulin in 55 healthy ( NGT ) , 30 impaired glucose-tolerant ( IGT ) , and 31 type 2 diabetic ( T2DM ) subjects .
	manualset3
84563	3	397938	14	13	NULL	0	NULL	oral glucose tolerance test ( OGTT ) data of insulin	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the different kinetics of the peptides , a mathematical model was necessary to analyze the oral glucose tolerance test ( OGTT ) data of insulin , C-peptide , and proinsulin in 55 healthy ( NGT ) , 30 impaired glucose-tolerant ( IGT ) , and 31 type 2 diabetic ( T2DM ) subjects .
	manualset3
84564	4	397938	14	13	NULL	NULL	NULL	oral glucose tolerance test ( OGTT ) data of C-peptide	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Given the different kinetics of the peptides , a mathematical model was necessary to analyze the oral glucose tolerance test ( OGTT ) data of insulin , C-peptide , and proinsulin in 55 healthy ( NGT ) , 30 impaired glucose-tolerant ( IGT ) , and 31 type 2 diabetic ( T2DM ) subjects .
	manualset3
84565	5	397938	14	13	NULL	0	NULL	oral glucose tolerance test ( OGTT ) data of proinsulin	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the different kinetics of the peptides , a mathematical model was necessary to analyze the oral glucose tolerance test ( OGTT ) data of insulin , C-peptide , and proinsulin in 55 healthy ( NGT ) , 30 impaired glucose-tolerant ( IGT ) , and 31 type 2 diabetic ( T2DM ) subjects .
	manualset3
84566	6	397938	14	13	NULL	0	NULL	55	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the different kinetics of the peptides , a mathematical model was necessary to analyze the oral glucose tolerance test ( OGTT ) data of insulin , C-peptide , and proinsulin in 55 healthy ( NGT ) , 30 impaired glucose-tolerant ( IGT ) , and 31 type 2 diabetic ( T2DM ) subjects .
	manualset3
84567	7	397938	14	13	NULL	0	NULL	healthy ( NGT ) subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the different kinetics of the peptides , a mathematical model was necessary to analyze the oral glucose tolerance test ( OGTT ) data of insulin , C-peptide , and proinsulin in 55 healthy ( NGT ) , 30 impaired glucose-tolerant ( IGT ) , and 31 type 2 diabetic ( T2DM ) subjects .
	manualset3
84568	8	397938	14	13	NULL	0	NULL	30	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the different kinetics of the peptides , a mathematical model was necessary to analyze the oral glucose tolerance test ( OGTT ) data of insulin , C-peptide , and proinsulin in 55 healthy ( NGT ) , 30 impaired glucose-tolerant ( IGT ) , and 31 type 2 diabetic ( T2DM ) subjects .
	manualset3
84569	9	397938	14	13	NULL	0	NULL	impaired glucose-tolerant ( IGT ) subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the different kinetics of the peptides , a mathematical model was necessary to analyze the oral glucose tolerance test ( OGTT ) data of insulin , C-peptide , and proinsulin in 55 healthy ( NGT ) , 30 impaired glucose-tolerant ( IGT ) , and 31 type 2 diabetic ( T2DM ) subjects .
	manualset3
84570	10	397938	14	13	NULL	0	NULL	31	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the different kinetics of the peptides , a mathematical model was necessary to analyze the oral glucose tolerance test ( OGTT ) data of insulin , C-peptide , and proinsulin in 55 healthy ( NGT ) , 30 impaired glucose-tolerant ( IGT ) , and 31 type 2 diabetic ( T2DM ) subjects .
	manualset3
84571	11	397938	14	13	NULL	0	NULL	type 2 diabetic ( T2DM ) subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the different kinetics of the peptides , a mathematical model was necessary to analyze the oral glucose tolerance test ( OGTT ) data of insulin , C-peptide , and proinsulin in 55 healthy ( NGT ) , 30 impaired glucose-tolerant ( IGT ) , and 31 type 2 diabetic ( T2DM ) subjects .
	manualset3
84572	1	397939	14	13	NULL	0	NULL	CALLA 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the fact that CALLA is completely modulated on the surface of lymphoid cells , we have employed pre-embedding immunogold techniques at electron-microscopical level and demonstrated that J5 monoclonal antibody ( MoAb ) - mediated modulation of CALLA expression on the lymphoblastic cell line NALM-6 is a specific , rapid process , closely resembling receptor-mediated endocytosis .
	manualset3
84573	2	397939	14	13	NULL	0	NULL	surface of lymphoid cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the fact that CALLA is completely modulated on the surface of lymphoid cells , we have employed pre-embedding immunogold techniques at electron-microscopical level and demonstrated that J5 monoclonal antibody ( MoAb ) - mediated modulation of CALLA expression on the lymphoblastic cell line NALM-6 is a specific , rapid process , closely resembling receptor-mediated endocytosis .
	manualset3
84574	3	397939	14	13	NULL	NULL	NULL	pre-embedding immunogold techniques  at electron-microscopical level	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Given the fact that CALLA is completely modulated on the surface of lymphoid cells , we have employed pre-embedding immunogold techniques at electron-microscopical level and demonstrated that J5 monoclonal antibody ( MoAb ) - mediated modulation of CALLA expression on the lymphoblastic cell line NALM-6 is a specific , rapid process , closely resembling receptor-mediated endocytosis .
	manualset3
84575	4	397939	14	13	NULL	0	NULL	J5 monoclonal antibody ( MoAb ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the fact that CALLA is completely modulated on the surface of lymphoid cells , we have employed pre-embedding immunogold techniques at electron-microscopical level and demonstrated that J5 monoclonal antibody ( MoAb ) - mediated modulation of CALLA expression on the lymphoblastic cell line NALM-6 is a specific , rapid process , closely resembling receptor-mediated endocytosis .
	manualset3
84576	5	397939	14	13	NULL	0	NULL	CALLA expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the fact that CALLA is completely modulated on the surface of lymphoid cells , we have employed pre-embedding immunogold techniques at electron-microscopical level and demonstrated that J5 monoclonal antibody ( MoAb ) - mediated modulation of CALLA expression on the lymphoblastic cell line NALM-6 is a specific , rapid process , closely resembling receptor-mediated endocytosis .
	manualset3
84577	6	397939	14	13	NULL	0	NULL	lymphoblastic cell line NALM-6	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the fact that CALLA is completely modulated on the surface of lymphoid cells , we have employed pre-embedding immunogold techniques at electron-microscopical level and demonstrated that J5 monoclonal antibody ( MoAb ) - mediated modulation of CALLA expression on the lymphoblastic cell line NALM-6 is a specific , rapid process , closely resembling receptor-mediated endocytosis .
	manualset3
84578	7	397939	14	13	NULL	0	NULL	receptor-mediated endocytosis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the fact that CALLA is completely modulated on the surface of lymphoid cells , we have employed pre-embedding immunogold techniques at electron-microscopical level and demonstrated that J5 monoclonal antibody ( MoAb ) - mediated modulation of CALLA expression on the lymphoblastic cell line NALM-6 is a specific , rapid process , closely resembling receptor-mediated endocytosis .
	manualset3
84580	2	397940	14	13	NULL	NULL	NULL	health care	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Given the imbalances and inefficiencies of market forces in health care , perverse incentives that have strengthened resistance to change , and secrecy when it comes to adverse event information , however , it is likely that policy initiatives will continue to play an important role in the transformation of the industry to more highly reliable , safer levels of care .
	manualset3
84677	3	397940	14	13	NULL	0	NULL	safer levels of care 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the imbalances and inefficiencies of market forces in health care , perverse incentives that have strengthened resistance to change , and secrecy when it comes to adverse event information , however , it is likely that policy initiatives will continue to play an important role in the transformation of the industry to more highly reliable , safer levels of care .
	manualset3
84678	4	397940	14	13	NULL	0	NULL	industry	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the imbalances and inefficiencies of market forces in health care , perverse incentives that have strengthened resistance to change , and secrecy when it comes to adverse event information , however , it is likely that policy initiatives will continue to play an important role in the transformation of the industry to more highly reliable , safer levels of care .
	manualset3
84773	1	397940	14	13	NULL	0	NULL	transformation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the imbalances and inefficiencies of market forces in health care , perverse incentives that have strengthened resistance to change , and secrecy when it comes to adverse event information , however , it is likely that policy initiatives will continue to play an important role in the transformation of the industry to more highly reliable , safer levels of care .
	manualset3
84581	1	397941	14	13	NULL	0	NULL	urolithiasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the influence of the composition of the urolithiasis for its treatment , we must insist on the collection of the greater number of samples for its analysis , although the epidemiologic data and the study of the urinary sediment can be used in the practice .
	manualset3
84582	2	397941	14	13	NULL	0	NULL	samples	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the influence of the composition of the urolithiasis for its treatment , we must insist on the collection of the greater number of samples for its analysis , although the epidemiologic data and the study of the urinary sediment can be used in the practice .
	manualset3
84583	3	397941	14	13	NULL	0	NULL	 analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the influence of the composition of the urolithiasis for its treatment , we must insist on the collection of the greater number of samples for its analysis , although the epidemiologic data and the study of the urinary sediment can be used in the practice .
	manualset3
84584	4	397941	14	13	NULL	0	NULL	 treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the influence of the composition of the urolithiasis for its treatment , we must insist on the collection of the greater number of samples for its analysis , although the epidemiologic data and the study of the urinary sediment can be used in the practice .
	manualset3
84585	5	397941	14	13	NULL	0	NULL	epidemiologic data 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the influence of the composition of the urolithiasis for its treatment , we must insist on the collection of the greater number of samples for its analysis , although the epidemiologic data and the study of the urinary sediment can be used in the practice .
	manualset3
84586	6	397941	14	13	NULL	0	NULL	study of the urinary sediment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the influence of the composition of the urolithiasis for its treatment , we must insist on the collection of the greater number of samples for its analysis , although the epidemiologic data and the study of the urinary sediment can be used in the practice .
	manualset3
84587	1	397942	14	13	NULL	NULL	NULL	Patient Protection and Affordable Care Act ( PPACA ) 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Given the passage of the Patient Protection and Affordable Care Act ( PPACA ) of 2010 , researchers and policy makers must agree on the model that best monitors and evaluates these new policy initiatives .
	manualset3
84588	2	397942	14	13	NULL	0	NULL	2010	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the passage of the Patient Protection and Affordable Care Act ( PPACA ) of 2010 , researchers and policy makers must agree on the model that best monitors and evaluates these new policy initiatives .
	manualset3
84589	3	397942	14	13	NULL	0	NULL	researchers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the passage of the Patient Protection and Affordable Care Act ( PPACA ) of 2010 , researchers and policy makers must agree on the model that best monitors and evaluates these new policy initiatives .
	manualset3
84590	4	397942	14	13	NULL	0	NULL	policy makers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the passage of the Patient Protection and Affordable Care Act ( PPACA ) of 2010 , researchers and policy makers must agree on the model that best monitors and evaluates these new policy initiatives .
	manualset3
84591	5	397942	14	13	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the passage of the Patient Protection and Affordable Care Act ( PPACA ) of 2010 , researchers and policy makers must agree on the model that best monitors and evaluates these new policy initiatives .
	manualset3
84592	6	397942	14	13	NULL	0	NULL	new policy initiatives	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the passage of the Patient Protection and Affordable Care Act ( PPACA ) of 2010 , researchers and policy makers must agree on the model that best monitors and evaluates these new policy initiatives .
	manualset3
84593	1	397943	14	13	NULL	0	NULL	glycyphyllin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the reported level of activity it is unlikely that glycyphyllin would provide direct antioxidant protection in tissues affected by oxidative stress .
	manualset3
84594	2	397943	14	13	NULL	0	NULL	antioxidant protection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the reported level of activity it is unlikely that glycyphyllin would provide direct antioxidant protection in tissues affected by oxidative stress .
	manualset3
84595	3	397943	14	13	NULL	0	NULL	tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the reported level of activity it is unlikely that glycyphyllin would provide direct antioxidant protection in tissues affected by oxidative stress .
	manualset3
84596	4	397943	14	13	NULL	0	NULL	oxidative stress	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Given the reported level of activity it is unlikely that glycyphyllin would provide direct antioxidant protection in tissues affected by oxidative stress .
	manualset3
84597	1	397944	14	13	NULL	0	NULL	wide variety of disease states	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Given their roles in such a wide variety of disease states , protein kinases are rapidly becoming extremely attractive targets for drug discovery , probably second only to heterotrimeric G protein-coupled receptors ( eg , angiotensin II ) .
	manualset3
84598	2	397944	14	13	NULL	NULL	NULL	protein kinases	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Given their roles in such a wide variety of disease states , protein kinases are rapidly becoming extremely attractive targets for drug discovery , probably second only to heterotrimeric G protein-coupled receptors ( eg , angiotensin II ) .
	manualset3
84599	3	397944	14	13	NULL	NULL	NULL	attractive targets	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Given their roles in such a wide variety of disease states , protein kinases are rapidly becoming extremely attractive targets for drug discovery , probably second only to heterotrimeric G protein-coupled receptors ( eg , angiotensin II ) .
	manualset3
84600	4	397944	14	13	NULL	0	NULL	drug discovery	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Given their roles in such a wide variety of disease states , protein kinases are rapidly becoming extremely attractive targets for drug discovery , probably second only to heterotrimeric G protein-coupled receptors ( eg , angiotensin II ) .
	manualset3
84601	5	397944	14	13	NULL	NULL	NULL	heterotrimeric G protein-coupled receptors	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Given their roles in such a wide variety of disease states , protein kinases are rapidly becoming extremely attractive targets for drug discovery , probably second only to heterotrimeric G protein-coupled receptors ( eg , angiotensin II ) .
	manualset3
84602	6	397944	14	13	NULL	0	NULL	angiotensin II 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Given their roles in such a wide variety of disease states , protein kinases are rapidly becoming extremely attractive targets for drug discovery , probably second only to heterotrimeric G protein-coupled receptors ( eg , angiotensin II ) .
	manualset3
84603	1	397945	14	13	NULL	0	NULL	Glasses	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	Glasses with a large laser effect : Nd-phosphate and Nd-fluorophosphate .
	manualset3
84604	2	397945	14	13	NULL	0	NULL	Nd-phosphate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Glasses with a large laser effect : Nd-phosphate and Nd-fluorophosphate .
	manualset3
84605	3	397945	14	13	NULL	0	NULL	Nd-fluorophosphate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Glasses with a large laser effect : Nd-phosphate and Nd-fluorophosphate .
	manualset3
84606	1	397946	14	13	NULL	0	NULL	Glatiramer acetate-specific T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Glatiramer acetate-specific T cells in the brain express T helper 2/3 cytokines and brain-derived neurotrophic factor in situ .
	manualset3
84607	2	397946	14	13	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Glatiramer acetate-specific T cells in the brain express T helper 2/3 cytokines and brain-derived neurotrophic factor in situ .
	manualset3
84608	3	397946	14	13	NULL	NULL	NULL	T helper 2/3 cytokines	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glatiramer acetate-specific T cells in the brain express T helper 2/3 cytokines and brain-derived neurotrophic factor in situ .
	manualset3
84610	4	397946	14	13	NULL	NULL	NULL	brain-derived neurotrophic factor 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glatiramer acetate-specific T cells in the brain express T helper 2/3 cytokines and brain-derived neurotrophic factor in situ .
	manualset3
84611	1	397947	14	13	NULL	0	NULL	Glaucoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Glaucoma in the developing world .
	manualset3
84612	2	397947	14	13	NULL	0	NULL	developing world	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Glaucoma in the developing world .
	manualset3
84613	1	397948	14	13	NULL	0	NULL	GlcN	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	GlcN completely abolished glycogen synthesis in the liver .
	manualset3
84614	2	397948	14	13	NULL	0	NULL	glycogen synthesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GlcN completely abolished glycogen synthesis in the liver .
	manualset3
84615	3	397948	14	13	NULL	0	NULL	liver 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	GlcN completely abolished glycogen synthesis in the liver .
	manualset3
84616	1	397949	14	13	NULL	NULL	NULL	Gleason grade	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gleason grade has been linked to a number of clinical end points , including clinical stage , progression to metastatic disease , and survival .
	manualset3
84617	2	397949	14	13	NULL	0	NULL	clinical end points	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gleason grade has been linked to a number of clinical end points , including clinical stage , progression to metastatic disease , and survival .
	manualset3
84618	3	397949	14	13	NULL	0	NULL	clinical stage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gleason grade has been linked to a number of clinical end points , including clinical stage , progression to metastatic disease , and survival .
	manualset3
84619	4	397949	14	13	NULL	0	NULL	progression to metastatic disease	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gleason grade has been linked to a number of clinical end points , including clinical stage , progression to metastatic disease , and survival .
	manualset3
84620	6	397949	14	13	NULL	0	NULL	survival 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gleason grade has been linked to a number of clinical end points , including clinical stage , progression to metastatic disease , and survival .
	manualset3
84621	1	397950	14	13	NULL	0	NULL	Glenohumeral range of motion deficits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Glenohumeral range of motion deficits and posterior shoulder tightness in throwers with pathologic internal impingement .
	manualset3
84622	2	397950	14	13	NULL	0	NULL	posterior shoulder tightness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Glenohumeral range of motion deficits and posterior shoulder tightness in throwers with pathologic internal impingement .
	manualset3
84623	3	397950	14	13	NULL	0	NULL	 throwers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Glenohumeral range of motion deficits and posterior shoulder tightness in throwers with pathologic internal impingement .
	manualset3
84624	4	397950	14	13	NULL	0	NULL	pathologic internal impingement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Glenohumeral range of motion deficits and posterior shoulder tightness in throwers with pathologic internal impingement .
	manualset3
84625	1	397951	14	13	NULL	NULL	NULL	Gli/Ci proteins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gli/Ci proteins possess a nuclear localization signal ( NLS ) and a nuclear export signal ( NES ) , both of which are key signatures for controlling nucleocytoplasmic shuttling .
	manualset3
84626	2	397951	14	13	NULL	0	NULL	nuclear localization signal ( NLS )	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gli/Ci proteins possess a nuclear localization signal ( NLS ) and a nuclear export signal ( NES ) , both of which are key signatures for controlling nucleocytoplasmic shuttling .
	manualset3
84627	3	397951	14	13	NULL	0	NULL	nuclear export signal ( NES )	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gli/Ci proteins possess a nuclear localization signal ( NLS ) and a nuclear export signal ( NES ) , both of which are key signatures for controlling nucleocytoplasmic shuttling .
	manualset3
84629	4	397951	14	13	NULL	NULL	NULL	nucleocytoplasmic shuttling	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gli/Ci proteins possess a nuclear localization signal ( NLS ) and a nuclear export signal ( NES ) , both of which are key signatures for controlling nucleocytoplasmic shuttling .
	manualset3
84630	1	397952	14	13	NULL	0	NULL	Glibenclamide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Glibenclamide and tetraethylammonium chloride ( TEA ) also did not influence the relaxation induced by the compounds .
	manualset3
84631	2	397952	14	13	NULL	0	NULL	tetraethylammonium chloride ( TEA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Glibenclamide and tetraethylammonium chloride ( TEA ) also did not influence the relaxation induced by the compounds .
	manualset3
84632	3	397952	14	13	NULL	0	NULL	relaxation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Glibenclamide and tetraethylammonium chloride ( TEA ) also did not influence the relaxation induced by the compounds .
	manualset3
84633	4	397952	14	13	NULL	0	NULL	compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Glibenclamide and tetraethylammonium chloride ( TEA ) also did not influence the relaxation induced by the compounds .
	manualset3
84634	1	397953	14	13	NULL	NULL	NULL	Gliomatosis cerebri is an infrequent tumor of neuroepithelial origin	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gliomatosis cerebri is an infrequent tumor of neuroepithelial origin presenting with deterioration of cognitive functions , behavioral and mental changes , motor weakness , headache , and seizures .
	manualset3
84636	3	397953	14	13	NULL	0	NULL	deterioration of cognitive functions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gliomatosis cerebri is an infrequent tumor of neuroepithelial origin presenting with deterioration of cognitive functions , behavioral and mental changes , motor weakness , headache , and seizures .
	manualset3
84637	4	397953	14	13	NULL	NULL	NULL	behavioral and mental changes	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gliomatosis cerebri is an infrequent tumor of neuroepithelial origin presenting with deterioration of cognitive functions , behavioral and mental changes , motor weakness , headache , and seizures .
	manualset3
84638	5	397953	14	13	NULL	0	NULL	motor weakness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gliomatosis cerebri is an infrequent tumor of neuroepithelial origin presenting with deterioration of cognitive functions , behavioral and mental changes , motor weakness , headache , and seizures .
	manualset3
84639	6	397953	14	13	NULL	0	NULL	headache	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gliomatosis cerebri is an infrequent tumor of neuroepithelial origin presenting with deterioration of cognitive functions , behavioral and mental changes , motor weakness , headache , and seizures .
	manualset3
84640	7	397953	14	13	NULL	0	NULL	seizures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gliomatosis cerebri is an infrequent tumor of neuroepithelial origin presenting with deterioration of cognitive functions , behavioral and mental changes , motor weakness , headache , and seizures .
	manualset3
84641	1	397954	14	13	NULL	0	NULL	Gliotoxin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Gliotoxin stimulates the apoptosis of human and rat hepatic stellate cells and enhances the resolution of liver fibrosis in rats .
	manualset3
84642	2	397954	14	13	NULL	NULL	NULL	apoptosis 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gliotoxin stimulates the apoptosis of human and rat hepatic stellate cells and enhances the resolution of liver fibrosis in rats .
	manualset3
84643	3	397954	14	13	NULL	NULL	NULL	human hepatic stellate cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gliotoxin stimulates the apoptosis of human and rat hepatic stellate cells and enhances the resolution of liver fibrosis in rats .
	manualset3
84644	4	397954	14	13	NULL	0	NULL	rat hepatic stellate cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Gliotoxin stimulates the apoptosis of human and rat hepatic stellate cells and enhances the resolution of liver fibrosis in rats .
	manualset3
84645	5	397954	14	13	NULL	0	NULL	liver fibrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gliotoxin stimulates the apoptosis of human and rat hepatic stellate cells and enhances the resolution of liver fibrosis in rats .
	manualset3
84646	6	397954	14	13	NULL	0	NULL	 rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Gliotoxin stimulates the apoptosis of human and rat hepatic stellate cells and enhances the resolution of liver fibrosis in rats .
	manualset3
84647	1	397955	14	13	NULL	0	NULL	Global analysis of the variations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Global analysis of the variations introduced on pyridine , pyrimidine and thiazole rings of this tricyclic system showed an increases of diuretic and natriuretic activities when the formal charge on N9a and C9b increases .
	manualset3
84648	2	397955	14	13	NULL	0	NULL	pyridine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Global analysis of the variations introduced on pyridine , pyrimidine and thiazole rings of this tricyclic system showed an increases of diuretic and natriuretic activities when the formal charge on N9a and C9b increases .
	manualset3
84649	3	397955	14	13	NULL	0	NULL	pyrimidine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Global analysis of the variations introduced on pyridine , pyrimidine and thiazole rings of this tricyclic system showed an increases of diuretic and natriuretic activities when the formal charge on N9a and C9b increases .
	manualset3
84650	4	397955	14	13	NULL	0	NULL	thiazole rings 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Global analysis of the variations introduced on pyridine , pyrimidine and thiazole rings of this tricyclic system showed an increases of diuretic and natriuretic activities when the formal charge on N9a and C9b increases .
	manualset3
84651	5	397955	14	13	NULL	NULL	NULL	N9a	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Global analysis of the variations introduced on pyridine , pyrimidine and thiazole rings of this tricyclic system showed an increases of diuretic and natriuretic activities when the formal charge on N9a and C9b increases .
	manualset3
84652	6	397955	14	13	NULL	NULL	NULL	C9b	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Global analysis of the variations introduced on pyridine , pyrimidine and thiazole rings of this tricyclic system showed an increases of diuretic and natriuretic activities when the formal charge on N9a and C9b increases .
	manualset3
84653	7	397955	14	13	NULL	0	NULL	diuretic activities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Global analysis of the variations introduced on pyridine , pyrimidine and thiazole rings of this tricyclic system showed an increases of diuretic and natriuretic activities when the formal charge on N9a and C9b increases .
	manualset3
84654	8	397955	14	13	NULL	0	NULL	natriuretic activities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Global analysis of the variations introduced on pyridine , pyrimidine and thiazole rings of this tricyclic system showed an increases of diuretic and natriuretic activities when the formal charge on N9a and C9b increases .
	manualset3
84655	1	397956	14	13	NULL	0	NULL	Global cooling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Global cooling after the eruption of Mount Pinatubo : a test of climate feedback by water vapor .
	manualset3
84656	2	397956	14	13	NULL	0	NULL	eruption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Global cooling after the eruption of Mount Pinatubo : a test of climate feedback by water vapor .
	manualset3
84657	3	397956	14	13	NULL	0	NULL	Mount Pinatubo	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Global cooling after the eruption of Mount Pinatubo : a test of climate feedback by water vapor .
	manualset3
84658	4	397956	14	13	NULL	0	NULL	climate	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Global cooling after the eruption of Mount Pinatubo : a test of climate feedback by water vapor .
	manualset3
84659	5	397956	14	13	NULL	0	NULL	water vapor 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Global cooling after the eruption of Mount Pinatubo : a test of climate feedback by water vapor .
	manualset3
84660	1	397957	14	13	NULL	0	NULL	Global left ventricular wall motion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Global left ventricular wall motion in patients with persisting or resolved thrombus was similar during follow-up .
	manualset3
84661	2	397957	14	13	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Global left ventricular wall motion in patients with persisting or resolved thrombus was similar during follow-up .
	manualset3
84662	3	397957	14	13	NULL	0	NULL	persisting or resolved thrombus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Global left ventricular wall motion in patients with persisting or resolved thrombus was similar during follow-up .
	manualset3
84663	4	397957	14	13	NULL	0	NULL	follow-up	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Global left ventricular wall motion in patients with persisting or resolved thrombus was similar during follow-up .
	manualset3
84664	1	397958	14	13	NULL	0	NULL	Global parsimony analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Global parsimony analysis recovers a monophyletic Bradoriida as the sister group to crown crustaceans .
	manualset3
84665	2	397958	14	13	NULL	0	NULL	monophyletic Bradoriida 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Global parsimony analysis recovers a monophyletic Bradoriida as the sister group to crown crustaceans .
	manualset3
84666	3	397958	14	13	NULL	0	NULL	sister group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Global parsimony analysis recovers a monophyletic Bradoriida as the sister group to crown crustaceans .
	manualset3
84667	4	397958	14	13	NULL	0	NULL	crown crustaceans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Global parsimony analysis recovers a monophyletic Bradoriida as the sister group to crown crustaceans .
	manualset3
84668	1	397959	14	13	NULL	0	NULL	Global theory	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Global theory and the nature of risk , Part I. How orthodox managed care stifles innovation .
	manualset3
84671	3	397959	14	13	NULL	NULL	NULL	orthodox	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Global theory and the nature of risk , Part I. How orthodox managed care stifles innovation .
	manualset3
84673	1	397960	14	13	NULL	NULL	NULL	Global Quality of Life	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Global Quality of Life slightly improved after masitinib therapy and did not predicted depression improvement .
	manualset3
84675	2	397960	14	13	NULL	NULL	NULL	masitinib therapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Global Quality of Life slightly improved after masitinib therapy and did not predicted depression improvement .
	manualset3
84676	3	397960	14	13	NULL	NULL	NULL	depression improvement 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Global Quality of Life slightly improved after masitinib therapy and did not predicted depression improvement .
	manualset3
84679	1	397961	14	13	NULL	0	NULL	 diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Some problems in the diagnosis , treatment and prevention of ischemic heart disease ) .
	manualset3
84680	2	397961	14	13	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Some problems in the diagnosis , treatment and prevention of ischemic heart disease ) .
	manualset3
84681	3	397961	14	13	NULL	0	NULL	prevention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Some problems in the diagnosis , treatment and prevention of ischemic heart disease ) .
	manualset3
84682	4	397961	14	13	NULL	0	NULL	 ischemic heart disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Some problems in the diagnosis , treatment and prevention of ischemic heart disease ) .
	manualset3
84689	1	397963	14	13	NULL	0	NULL	Glomerular charge and size selectivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Glomerular charge and size selectivity assessed by changes in salt intake in type 2 diabetic patients .
	manualset3
84690	2	397963	14	13	NULL	NULL	NULL	salt intake	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glomerular charge and size selectivity assessed by changes in salt intake in type 2 diabetic patients .
	manualset3
84691	4	397963	14	13	NULL	NULL	NULL	 type 2 diabetic patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glomerular charge and size selectivity assessed by changes in salt intake in type 2 diabetic patients .
	manualset3
84693	1	397964	14	13	NULL	0	NULL	Glucagon-induced changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Glucagon-induced changes in fructose 2 , 6-bisphosphate and 6-phosphofructo-2-kinase in cultured rat foetal hepatocytes .
	manualset3
84694	2	397964	14	13	NULL	NULL	NULL	fructose 2 , 6-bisphosphate	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glucagon-induced changes in fructose 2 , 6-bisphosphate and 6-phosphofructo-2-kinase in cultured rat foetal hepatocytes .
	manualset3
84695	3	397964	14	13	NULL	0	NULL	6-phosphofructo-2-kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Glucagon-induced changes in fructose 2 , 6-bisphosphate and 6-phosphofructo-2-kinase in cultured rat foetal hepatocytes .
	manualset3
84696	4	397964	14	13	NULL	0	NULL	cultured rat foetal hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Glucagon-induced changes in fructose 2 , 6-bisphosphate and 6-phosphofructo-2-kinase in cultured rat foetal hepatocytes .
	manualset3
84697	1	397965	14	13	NULL	NULL	NULL	Glucocorticoids 	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glucocorticoids , the end-products of the hypothalamic-pituitary - adrenal ( HPA ) axis , influence the functions of virtually all organs and tissues through the nuclear glucocorticoid receptor ( GR ) .
	manualset3
84698	2	397965	14	13	NULL	0	NULL	hypothalamic-pituitary - adrenal ( HPA ) axis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Glucocorticoids , the end-products of the hypothalamic-pituitary - adrenal ( HPA ) axis , influence the functions of virtually all organs and tissues through the nuclear glucocorticoid receptor ( GR ) .
	manualset3
84700	3	397965	14	13	NULL	NULL	NULL	 functions of virtually all organs and tissues 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glucocorticoids , the end-products of the hypothalamic-pituitary - adrenal ( HPA ) axis , influence the functions of virtually all organs and tissues through the nuclear glucocorticoid receptor ( GR ) .
	manualset3
84702	4	397965	14	13	NULL	NULL	NULL	nuclear glucocorticoid receptor ( GR ) 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glucocorticoids , the end-products of the hypothalamic-pituitary - adrenal ( HPA ) axis , influence the functions of virtually all organs and tissues through the nuclear glucocorticoid receptor ( GR ) .
	manualset3
84703	1	397966	14	13	NULL	NULL	NULL	Glucocorticoids	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glucocorticoids acting through the glucocorticoid receptor ( GR ) inhibit TNF-induced lethal inflammation .
	manualset3
84704	2	397966	14	13	NULL	0	NULL	glucocorticoid receptor ( GR ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Glucocorticoids acting through the glucocorticoid receptor ( GR ) inhibit TNF-induced lethal inflammation .
	manualset3
84705	3	397966	14	13	NULL	NULL	NULL	TNF-induced lethal inflammation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glucocorticoids acting through the glucocorticoid receptor ( GR ) inhibit TNF-induced lethal inflammation .
	manualset3
84707	1	397967	14	13	NULL	NULL	NULL	Glucose	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glucose and xylose were co-utilized , and transport studies suggested that there was a common transport system for both sugars .
	manualset3
84708	2	397967	14	13	NULL	NULL	NULL	xylose	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glucose and xylose were co-utilized , and transport studies suggested that there was a common transport system for both sugars .
	manualset3
84709	3	397967	14	13	NULL	0	NULL	transport studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Glucose and xylose were co-utilized , and transport studies suggested that there was a common transport system for both sugars .
	manualset3
84710	4	397967	14	13	NULL	0	NULL	common transport system	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Glucose and xylose were co-utilized , and transport studies suggested that there was a common transport system for both sugars .
	manualset3
84711	5	397967	14	13	NULL	NULL	NULL	both sugars	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glucose and xylose were co-utilized , and transport studies suggested that there was a common transport system for both sugars .
	manualset3
84712	1	397968	14	13	NULL	NULL	NULL	Glucose 	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glucose had no such effect , although this carbohydrate and L-proline were transported in similar fashions .
	manualset3
84713	2	397968	14	13	NULL	NULL	NULL	carbohydrate	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glucose had no such effect , although this carbohydrate and L-proline were transported in similar fashions .
	manualset3
84714	3	397968	14	13	NULL	NULL	NULL	L-proline	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glucose had no such effect , although this carbohydrate and L-proline were transported in similar fashions .
	manualset3
84715	4	397968	14	13	NULL	0	NULL	 transported in similar fashions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Glucose had no such effect , although this carbohydrate and L-proline were transported in similar fashions .
	manualset3
84716	1	397969	14	13	NULL	0	NULL	Glucose intolerance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Glucose intolerance was associated with the risk of gallstones independent of obesity .
	manualset3
84717	2	397969	14	13	NULL	0	NULL	risk of gallstones	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Glucose intolerance was associated with the risk of gallstones independent of obesity .
	manualset3
84718	3	397969	14	13	NULL	0	NULL	obesity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Glucose intolerance was associated with the risk of gallstones independent of obesity .
	manualset3
84719	1	397970	14	13	NULL	0	NULL	Glucose metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Glucose metabolism , which was also studied for the plaque samples , was not significantly affected by presence of any of the 2 detergents , indicating that the amounts of xylitol in toothpastes were presumably too low to give clinical significant effects , even when mild detergents are used .
	manualset3
84720	2	397970	14	13	NULL	0	NULL	plaque samples	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Glucose metabolism , which was also studied for the plaque samples , was not significantly affected by presence of any of the 2 detergents , indicating that the amounts of xylitol in toothpastes were presumably too low to give clinical significant effects , even when mild detergents are used .
	manualset3
84721	3	397970	14	13	NULL	0	NULL	2	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Glucose metabolism , which was also studied for the plaque samples , was not significantly affected by presence of any of the 2 detergents , indicating that the amounts of xylitol in toothpastes were presumably too low to give clinical significant effects , even when mild detergents are used .
	manualset3
84722	4	397970	14	13	NULL	0	NULL	detergents	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	Glucose metabolism , which was also studied for the plaque samples , was not significantly affected by presence of any of the 2 detergents , indicating that the amounts of xylitol in toothpastes were presumably too low to give clinical significant effects , even when mild detergents are used .
	manualset3
84723	5	397970	14	13	NULL	0	NULL	xylitol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Glucose metabolism , which was also studied for the plaque samples , was not significantly affected by presence of any of the 2 detergents , indicating that the amounts of xylitol in toothpastes were presumably too low to give clinical significant effects , even when mild detergents are used .
	manualset3
84724	6	397970	14	13	NULL	0	NULL	toothpastes	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	Glucose metabolism , which was also studied for the plaque samples , was not significantly affected by presence of any of the 2 detergents , indicating that the amounts of xylitol in toothpastes were presumably too low to give clinical significant effects , even when mild detergents are used .
	manualset3
84726	8	397970	14	13	NULL	NULL	NULL	clinical significant effects 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glucose metabolism , which was also studied for the plaque samples , was not significantly affected by presence of any of the 2 detergents , indicating that the amounts of xylitol in toothpastes were presumably too low to give clinical significant effects , even when mild detergents are used .
	manualset3
84727	9	397970	14	13	NULL	0	NULL	mild detergents	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	Glucose metabolism , which was also studied for the plaque samples , was not significantly affected by presence of any of the 2 detergents , indicating that the amounts of xylitol in toothpastes were presumably too low to give clinical significant effects , even when mild detergents are used .
	manualset3
84729	1	397971	14	13	NULL	NULL	NULL	study 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Some progress in study on mind and brain ) .
	manualset3
84730	2	397971	14	13	NULL	NULL	NULL	mind	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Some progress in study on mind and brain ) .
	manualset3
84731	3	397971	14	13	NULL	NULL	NULL	brain	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Some progress in study on mind and brain ) .
	manualset3
84732	1	397972	14	13	NULL	0	NULL	Glucose tolerance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Glucose tolerance improved after the barley meal , with the peak OGTT plasma glucose concentration being 0.7 mmol/L lower than that after the rice meal ( 7.7 + / - 0.4 v 8.4 + / - 0.3 mmol/L , P & lt ; .05 ) .
	manualset3
84733	2	397972	14	13	NULL	0	NULL	barley meal	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Glucose tolerance improved after the barley meal , with the peak OGTT plasma glucose concentration being 0.7 mmol/L lower than that after the rice meal ( 7.7 + / - 0.4 v 8.4 + / - 0.3 mmol/L , P & lt ; .05 ) .
	manualset3
84734	3	397972	14	13	NULL	0	NULL	peak OGTT plasma glucose concentration 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Glucose tolerance improved after the barley meal , with the peak OGTT plasma glucose concentration being 0.7 mmol/L lower than that after the rice meal ( 7.7 + / - 0.4 v 8.4 + / - 0.3 mmol/L , P & lt ; .05 ) .
	manualset3
84735	4	397972	14	13	NULL	0	NULL	0.7 mmol/L 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Glucose tolerance improved after the barley meal , with the peak OGTT plasma glucose concentration being 0.7 mmol/L lower than that after the rice meal ( 7.7 + / - 0.4 v 8.4 + / - 0.3 mmol/L , P & lt ; .05 ) .
	manualset3
84736	5	397972	14	13	NULL	0	NULL	rice meal	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Glucose tolerance improved after the barley meal , with the peak OGTT plasma glucose concentration being 0.7 mmol/L lower than that after the rice meal ( 7.7 + / - 0.4 v 8.4 + / - 0.3 mmol/L , P & lt ; .05 ) .
	manualset3
84737	6	397972	14	13	NULL	NULL	NULL	7.7 + / - 0.4 v 8.4 + / - 0.3 mmol/L , P & lt ; .05 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glucose tolerance improved after the barley meal , with the peak OGTT plasma glucose concentration being 0.7 mmol/L lower than that after the rice meal ( 7.7 + / - 0.4 v 8.4 + / - 0.3 mmol/L , P & lt ; .05 ) .
	manualset3
84738	1	397973	14	13	NULL	0	NULL	Glutamate-gated channels 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamate-gated channels mediate fundamental brain processes , yet the mechanisms by which the neurotransmitter controls channel activation are incompletely understood .
	manualset3
84739	2	397973	14	13	NULL	0	NULL	fundamental brain processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamate-gated channels mediate fundamental brain processes , yet the mechanisms by which the neurotransmitter controls channel activation are incompletely understood .
	manualset3
84740	3	397973	14	13	NULL	0	NULL	mechanisms 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamate-gated channels mediate fundamental brain processes , yet the mechanisms by which the neurotransmitter controls channel activation are incompletely understood .
	manualset3
84741	4	397973	14	13	NULL	0	NULL	neurotransmitter controls channel activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamate-gated channels mediate fundamental brain processes , yet the mechanisms by which the neurotransmitter controls channel activation are incompletely understood .
	manualset3
84742	1	397974	14	13	NULL	0	NULL	Glutamate dehydrogenase ( GDH ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamate dehydrogenase ( GDH ) is a homohexameric enzyme that catalyzes the reversible oxidative deamination of l-glutamate to 2-oxoglutarate .
	manualset3
84743	2	397974	14	13	NULL	0	NULL	homohexameric enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamate dehydrogenase ( GDH ) is a homohexameric enzyme that catalyzes the reversible oxidative deamination of l-glutamate to 2-oxoglutarate .
	manualset3
84744	3	397974	14	13	NULL	NULL	NULL	reversible oxidative deamination	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glutamate dehydrogenase ( GDH ) is a homohexameric enzyme that catalyzes the reversible oxidative deamination of l-glutamate to 2-oxoglutarate .
	manualset3
84745	4	397974	14	13	NULL	NULL	NULL	l-glutamate	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glutamate dehydrogenase ( GDH ) is a homohexameric enzyme that catalyzes the reversible oxidative deamination of l-glutamate to 2-oxoglutarate .
	manualset3
84746	5	397974	14	13	NULL	NULL	NULL	2-oxoglutarate	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glutamate dehydrogenase ( GDH ) is a homohexameric enzyme that catalyzes the reversible oxidative deamination of l-glutamate to 2-oxoglutarate .
	manualset3
84752	1	397976	14	13	NULL	NULL	NULL	Glutamate	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glutamate was oxidized via the tricarboxylic acid cycle .
	manualset3
84753	2	397976	14	13	NULL	0	NULL	oxidized	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamate was oxidized via the tricarboxylic acid cycle .
	manualset3
84754	3	397976	14	13	NULL	0	NULL	tricarboxylic acid cycle	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamate was oxidized via the tricarboxylic acid cycle .
	manualset3
84755	1	397977	14	13	NULL	0	NULL	Glutamatergic medications	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamatergic medications for the treatment of drug and behavioral addictions .
	manualset3
84756	2	397977	14	13	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamatergic medications for the treatment of drug and behavioral addictions .
	manualset3
84757	3	397977	14	13	NULL	0	NULL	drug and behavioral addictions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Glutamatergic medications for the treatment of drug and behavioral addictions .
	manualset3
84758	1	397978	14	13	NULL	NULL	NULL	Glutathione effects	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glutathione effects on toxicity and uptake of mercuric chloride and sodium arsenite in rabbit renal cortical slices .
	manualset3
84759	2	397978	14	13	NULL	0	NULL	 toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Glutathione effects on toxicity and uptake of mercuric chloride and sodium arsenite in rabbit renal cortical slices .
	manualset3
84760	3	397978	14	13	NULL	0	NULL	mercuric chloride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Glutathione effects on toxicity and uptake of mercuric chloride and sodium arsenite in rabbit renal cortical slices .
	manualset3
84761	4	397978	14	13	NULL	0	NULL	sodium arsenite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Glutathione effects on toxicity and uptake of mercuric chloride and sodium arsenite in rabbit renal cortical slices .
	manualset3
85429	5	397978	14	13	NULL	0	NULL	rabbit renal cortical slices	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Glutathione effects on toxicity and uptake of mercuric chloride and sodium arsenite in rabbit renal cortical slices .
	manualset3
85430	6	397978	14	13	NULL	0	NULL	uptake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Glutathione effects on toxicity and uptake of mercuric chloride and sodium arsenite in rabbit renal cortical slices .
	manualset3
84762	1	397979	14	13	NULL	NULL	NULL	Glycan-modifying bacteria-derived soluble factors	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glycan-modifying bacteria-derived soluble factors from Bacteroides thetaiotaomicron and Lactobacillus casei inhibit rotavirus infection in human intestinal cells .
	manualset3
84763	2	397979	14	13	NULL	0	NULL	Bacteroides thetaiotaomicron	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycan-modifying bacteria-derived soluble factors from Bacteroides thetaiotaomicron and Lactobacillus casei inhibit rotavirus infection in human intestinal cells .
	manualset3
84764	3	397979	14	13	NULL	0	NULL	Lactobacillus casei	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycan-modifying bacteria-derived soluble factors from Bacteroides thetaiotaomicron and Lactobacillus casei inhibit rotavirus infection in human intestinal cells .
	manualset3
84765	4	397979	14	13	NULL	0	NULL	rotavirus infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycan-modifying bacteria-derived soluble factors from Bacteroides thetaiotaomicron and Lactobacillus casei inhibit rotavirus infection in human intestinal cells .
	manualset3
84766	5	397979	14	13	NULL	0	NULL	human intestinal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycan-modifying bacteria-derived soluble factors from Bacteroides thetaiotaomicron and Lactobacillus casei inhibit rotavirus infection in human intestinal cells .
	manualset3
84767	1	397980	14	13	NULL	NULL	NULL	Glycans	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glycans released by peptide N-glycosidase were resolved by Bio-Gel P-4 gel filtration into two fractions : a low molecular mass mannose-rich fraction and a high molecular mass galactose and N-acetylglucosamine-rich fraction .
	manualset3
84768	2	397980	14	13	NULL	0	NULL	peptide N-glycosidase	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycans released by peptide N-glycosidase were resolved by Bio-Gel P-4 gel filtration into two fractions : a low molecular mass mannose-rich fraction and a high molecular mass galactose and N-acetylglucosamine-rich fraction .
	manualset3
84769	3	397980	14	13	NULL	0	NULL	Bio-Gel P-4 gel filtration	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycans released by peptide N-glycosidase were resolved by Bio-Gel P-4 gel filtration into two fractions : a low molecular mass mannose-rich fraction and a high molecular mass galactose and N-acetylglucosamine-rich fraction .
	manualset3
84770	4	397980	14	13	NULL	0	NULL	two fractions	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycans released by peptide N-glycosidase were resolved by Bio-Gel P-4 gel filtration into two fractions : a low molecular mass mannose-rich fraction and a high molecular mass galactose and N-acetylglucosamine-rich fraction .
	manualset3
84771	5	397980	14	13	NULL	NULL	NULL	a low molecular mass mannose-rich fraction 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glycans released by peptide N-glycosidase were resolved by Bio-Gel P-4 gel filtration into two fractions : a low molecular mass mannose-rich fraction and a high molecular mass galactose and N-acetylglucosamine-rich fraction .
	manualset3
84772	6	397980	14	13	NULL	0	NULL	 a high molecular mass galactose and N-acetylglucosamine-rich fraction	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycans released by peptide N-glycosidase were resolved by Bio-Gel P-4 gel filtration into two fractions : a low molecular mass mannose-rich fraction and a high molecular mass galactose and N-acetylglucosamine-rich fraction .
	manualset3
84876	1	397981	14	13	NULL	0	NULL	Glycerol kinase deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycerol kinase deficiency : compartmental considerations regarding pathogenesis and clinical heterogeneity .
	manualset3
84877	2	397981	14	13	NULL	0	NULL	pathogenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycerol kinase deficiency : compartmental considerations regarding pathogenesis and clinical heterogeneity .
	manualset3
84878	3	397981	14	13	NULL	0	NULL	clinical heterogeneity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycerol kinase deficiency : compartmental considerations regarding pathogenesis and clinical heterogeneity .
	manualset3
84879	1	397982	14	13	NULL	0	NULL	Glycoalkaloids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycoalkaloids are involved in the resistance of potatoes to pathogens and pests , but they also have implications for human health and nutrition .
	manualset3
84880	2	397982	14	13	NULL	NULL	NULL	resistance of potatoes	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glycoalkaloids are involved in the resistance of potatoes to pathogens and pests , but they also have implications for human health and nutrition .
	manualset3
84881	3	397982	14	13	NULL	0	NULL	pathogens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycoalkaloids are involved in the resistance of potatoes to pathogens and pests , but they also have implications for human health and nutrition .
	manualset3
84882	4	397982	14	13	NULL	NULL	NULL	pests	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glycoalkaloids are involved in the resistance of potatoes to pathogens and pests , but they also have implications for human health and nutrition .
	manualset3
84883	5	397982	14	13	NULL	NULL	NULL	human health	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glycoalkaloids are involved in the resistance of potatoes to pathogens and pests , but they also have implications for human health and nutrition .
	manualset3
84884	6	397982	14	13	NULL	0	NULL	nutrition	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycoalkaloids are involved in the resistance of potatoes to pathogens and pests , but they also have implications for human health and nutrition .
	manualset3
84885	1	397983	14	13	NULL	NULL	NULL	Glycolipid-protein interaction	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glycolipid-protein interaction in the mechanism of signal transduction : studies with a photoactivable ganglioside analog .
	manualset3
84886	2	397983	14	13	NULL	0	NULL	mechanism of signal transduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycolipid-protein interaction in the mechanism of signal transduction : studies with a photoactivable ganglioside analog .
	manualset3
84887	3	397983	14	13	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycolipid-protein interaction in the mechanism of signal transduction : studies with a photoactivable ganglioside analog .
	manualset3
84888	4	397983	14	13	NULL	0	NULL	photoactivable ganglioside analog	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycolipid-protein interaction in the mechanism of signal transduction : studies with a photoactivable ganglioside analog .
	manualset3
84889	1	397984	14	13	NULL	0	NULL	Glycolipids	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycolipids with gluco stereochemistry are the most prevalent .
	manualset3
84890	2	397984	14	13	NULL	0	NULL	gluco stereochemistry	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycolipids with gluco stereochemistry are the most prevalent .
	manualset3
84891	1	397985	14	13	NULL	0	NULL	Glycophorin A 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycophorin A is specific for the erythroid lineage of cells , and leukocytes have a major sialoglycoprotein , also called leukosialin or sialophorin .
	manualset3
84892	2	397985	14	13	NULL	0	NULL	erythroid lineage of cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycophorin A is specific for the erythroid lineage of cells , and leukocytes have a major sialoglycoprotein , also called leukosialin or sialophorin .
	manualset3
84893	3	397985	14	13	NULL	0	NULL	leukocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycophorin A is specific for the erythroid lineage of cells , and leukocytes have a major sialoglycoprotein , also called leukosialin or sialophorin .
	manualset3
84894	4	397985	14	13	NULL	0	NULL	major sialoglycoprotein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycophorin A is specific for the erythroid lineage of cells , and leukocytes have a major sialoglycoprotein , also called leukosialin or sialophorin .
	manualset3
84895	5	397985	14	13	NULL	0	NULL	leukosialin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycophorin A is specific for the erythroid lineage of cells , and leukocytes have a major sialoglycoprotein , also called leukosialin or sialophorin .
	manualset3
84896	6	397985	14	13	NULL	0	NULL	sialophorin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycophorin A is specific for the erythroid lineage of cells , and leukocytes have a major sialoglycoprotein , also called leukosialin or sialophorin .
	manualset3
84897	1	397986	14	13	NULL	0	NULL	Glycoprotein biosynthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycoprotein biosynthesis in liver mitochondria .
	manualset3
84898	2	397986	14	13	NULL	NULL	NULL	 liver mitochondria	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glycoprotein biosynthesis in liver mitochondria .
	manualset3
84899	1	397987	14	13	NULL	NULL	NULL	Glycoproteins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glycoproteins synthesized in SCO cells are released into the ventricular CSF where they aggregate , in a highly ordered fashion , forming an elongated supramacromolecular structure known as the Reissner 's fiber ( RF ) .
	manualset3
84900	2	397987	14	13	NULL	0	NULL	SCO cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycoproteins synthesized in SCO cells are released into the ventricular CSF where they aggregate , in a highly ordered fashion , forming an elongated supramacromolecular structure known as the Reissner 's fiber ( RF ) .
	manualset3
84901	3	397987	14	13	NULL	NULL	NULL	ventricular CSF	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glycoproteins synthesized in SCO cells are released into the ventricular CSF where they aggregate , in a highly ordered fashion , forming an elongated supramacromolecular structure known as the Reissner 's fiber ( RF ) .
	manualset3
84902	4	397987	14	13	NULL	NULL	NULL	elongated supramacromolecular structure	AnatomicalPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Glycoproteins synthesized in SCO cells are released into the ventricular CSF where they aggregate , in a highly ordered fashion , forming an elongated supramacromolecular structure known as the Reissner 's fiber ( RF ) .
	manualset3
85431	5	397987	14	13	NULL	0	NULL	Reissner 's fiber ( RF )	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycoproteins synthesized in SCO cells are released into the ventricular CSF where they aggregate , in a highly ordered fashion , forming an elongated supramacromolecular structure known as the Reissner 's fiber ( RF ) .
	manualset3
84903	1	397988	14	13	NULL	0	NULL	Glycosylation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycosylation and high-level secretion of human tumor necrosis factor-beta in recombinant baculovirus-infected insect cells .
	manualset3
84904	2	397988	14	13	NULL	0	NULL	secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycosylation and high-level secretion of human tumor necrosis factor-beta in recombinant baculovirus-infected insect cells .
	manualset3
84905	3	397988	14	13	NULL	0	NULL	 human tumor necrosis factor-beta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycosylation and high-level secretion of human tumor necrosis factor-beta in recombinant baculovirus-infected insect cells .
	manualset3
84906	4	397988	14	13	NULL	0	NULL	recombinant baculovirus-infected insect cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycosylation and high-level secretion of human tumor necrosis factor-beta in recombinant baculovirus-infected insect cells .
	manualset3
84907	1	397989	14	13	NULL	0	NULL	GnRH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	GnRH levels were determined at various times during an estrogen/progesterone ( E/P ) - induced LH surge .
	manualset3
84908	2	397989	14	13	NULL	NULL	NULL	estrogen/progesterone ( E/P ) - induced LH surge	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	GnRH levels were determined at various times during an estrogen/progesterone ( E/P ) - induced LH surge .
	manualset3
84910	1	397990	14	13	NULL	NULL	NULL	simple flow reactor	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Go with the flow : A simple flow reactor has been developed to accommodate highly absorbing ( RuL ( 3 ) ) ( 2 + ) photosensitizers for light-starved photoredox reactions .
	manualset3
84911	2	397990	14	13	NULL	0	NULL	( RuL ( 3 ) ) ( 2 + ) photosensitizers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Go with the flow : A simple flow reactor has been developed to accommodate highly absorbing ( RuL ( 3 ) ) ( 2 + ) photosensitizers for light-starved photoredox reactions .
	manualset3
84912	3	397990	14	13	NULL	0	NULL	light-starved photoredox reactions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Go with the flow : A simple flow reactor has been developed to accommodate highly absorbing ( RuL ( 3 ) ) ( 2 + ) photosensitizers for light-starved photoredox reactions .
	manualset3
84913	1	397991	14	13	NULL	0	NULL	Goals of therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Goals of therapy are different in lower risk patients than in higher risk .
	manualset3
84914	2	397991	14	13	NULL	0	NULL	lower risk patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Goals of therapy are different in lower risk patients than in higher risk .
	manualset3
84915	3	397991	14	13	NULL	0	NULL	higher risk patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Goals of therapy are different in lower risk patients than in higher risk .
	manualset3
84916	1	397992	14	13	NULL	0	NULL	Goals of treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Goals of treatment involve improving hypotension without excessive supine hypertension , relieving orthostatic symptoms , and improving standing time .
	manualset3
84917	2	397992	14	13	NULL	NULL	NULL	improving hypotension	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Goals of treatment involve improving hypotension without excessive supine hypertension , relieving orthostatic symptoms , and improving standing time .
	manualset3
84918	3	397992	14	13	NULL	NULL	NULL	supine hypertension	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Goals of treatment involve improving hypotension without excessive supine hypertension , relieving orthostatic symptoms , and improving standing time .
	manualset3
84919	4	397992	14	13	NULL	NULL	NULL	orthostatic symptoms	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Goals of treatment involve improving hypotension without excessive supine hypertension , relieving orthostatic symptoms , and improving standing time .
	manualset3
84920	5	397992	14	13	NULL	NULL	NULL	standing time	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Goals of treatment involve improving hypotension without excessive supine hypertension , relieving orthostatic symptoms , and improving standing time .
	manualset3
84921	1	397993	14	13	NULL	NULL	NULL	Alkaline	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Alkaline earth chelates from hydrolytically cleavable chelate constituents , I. On the calcium chelate of the N-glucoside of dimethylamino-alpha , alpha ' - dicarboxylic acid ( iminodiacetic acid ) ) .
	manualset3
84922	4	397993	14	13	NULL	NULL	NULL	hydrolytically cleavable chelate constituents	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Alkaline earth chelates from hydrolytically cleavable chelate constituents , I. On the calcium chelate of the N-glucoside of dimethylamino-alpha , alpha ' - dicarboxylic acid ( iminodiacetic acid ) ) .
	manualset3
85009	3	397993	14	13	NULL	0	NULL	calcium chelate of the N-glucoside of dimethylamino-alpha , alpha ' - dicarboxylic acid ( iminodiacetic acid ) )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Alkaline earth chelates from hydrolytically cleavable chelate constituents , I. On the calcium chelate of the N-glucoside of dimethylamino-alpha , alpha ' - dicarboxylic acid ( iminodiacetic acid ) ) .
	manualset3
85270	2	397993	14	13	NULL	0	NULL	chelates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Alkaline earth chelates from hydrolytically cleavable chelate constituents , I. On the calcium chelate of the N-glucoside of dimethylamino-alpha , alpha ' - dicarboxylic acid ( iminodiacetic acid ) ) .
	manualset3
85010	1	397994	14	13	NULL	0	NULL	Spectrophotometric determination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Spectrophotometric determination of tabletted allacil , methylthiouracil and hexamidine ) .
	manualset3
85011	2	397994	14	13	NULL	0	NULL	tabletted allacil	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Spectrophotometric determination of tabletted allacil , methylthiouracil and hexamidine ) .
	manualset3
85012	3	397994	14	13	NULL	0	NULL	methylthiouracil	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Spectrophotometric determination of tabletted allacil , methylthiouracil and hexamidine ) .
	manualset3
85013	4	397994	14	13	NULL	0	NULL	hexamidine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Spectrophotometric determination of tabletted allacil , methylthiouracil and hexamidine ) .
	manualset3
85014	1	397995	14	13	NULL	0	NULL	Gold phosphides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Gold phosphides show unique optical or semiconductor properties and there are extensive high technology applications , e.g. in laser diodes , etc. .
	manualset3
85015	2	397995	14	13	NULL	NULL	NULL	high technology applications	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gold phosphides show unique optical or semiconductor properties and there are extensive high technology applications , e.g. in laser diodes , etc. .
	manualset3
85016	3	397995	14	13	NULL	NULL	NULL	laser diodes	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gold phosphides show unique optical or semiconductor properties and there are extensive high technology applications , e.g. in laser diodes , etc. .
	manualset3
85017	1	397996	14	13	NULL	0	NULL	Gonadal dysgenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gonadal dysgenesis is an infrequent cause for primary amenorrhoea .
	manualset3
85018	2	397996	14	13	NULL	0	NULL	primary amenorrhoea	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Gonadal dysgenesis is an infrequent cause for primary amenorrhoea .
	manualset3
85019	1	397997	14	13	NULL	NULL	NULL	Gonadal function	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gonadal function in young women with Down syndrome .
	manualset3
85020	2	397997	14	13	NULL	0	NULL	young women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Gonadal function in young women with Down syndrome .
	manualset3
85021	3	397997	14	13	NULL	0	NULL	Down syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Gonadal function in young women with Down syndrome .
	manualset3
85022	1	397998	14	13	NULL	0	NULL	Gonadosomatic index ( GSI )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gonadosomatic index ( GSI ) , sperm quality , plasma sex steroids ( 11-keto testosterone ( 11-KT ) ; testosterone ( T ) ; estradiol-17beta ( E2 ) ) were evaluated on 10 to 24 fish fed on each diet .
	manualset3
85023	2	397998	14	13	NULL	0	NULL	sperm quality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gonadosomatic index ( GSI ) , sperm quality , plasma sex steroids ( 11-keto testosterone ( 11-KT ) ; testosterone ( T ) ; estradiol-17beta ( E2 ) ) were evaluated on 10 to 24 fish fed on each diet .
	manualset3
85024	3	397998	14	13	NULL	0	NULL	 plasma sex steroids ( 11-keto testosterone ( 11-KT ) ; testosterone ( T ) ; estradiol-17beta ( E2 ) )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Gonadosomatic index ( GSI ) , sperm quality , plasma sex steroids ( 11-keto testosterone ( 11-KT ) ; testosterone ( T ) ; estradiol-17beta ( E2 ) ) were evaluated on 10 to 24 fish fed on each diet .
	manualset3
85025	4	397998	14	13	NULL	NULL	NULL	10 to 24	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gonadosomatic index ( GSI ) , sperm quality , plasma sex steroids ( 11-keto testosterone ( 11-KT ) ; testosterone ( T ) ; estradiol-17beta ( E2 ) ) were evaluated on 10 to 24 fish fed on each diet .
	manualset3
85026	5	397998	14	13	NULL	NULL	NULL	fish fed on each diet 	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gonadosomatic index ( GSI ) , sperm quality , plasma sex steroids ( 11-keto testosterone ( 11-KT ) ; testosterone ( T ) ; estradiol-17beta ( E2 ) ) were evaluated on 10 to 24 fish fed on each diet .
	manualset3
85028	1	397999	14	13	NULL	0	NULL	Gonadotrophin pulsatility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gonadotrophin pulsatility in girls with the Turner syndrome : modulation by exogenous sex steroids .
	manualset3
85029	2	397999	14	13	NULL	0	NULL	girls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Gonadotrophin pulsatility in girls with the Turner syndrome : modulation by exogenous sex steroids .
	manualset3
85030	3	397999	14	13	NULL	0	NULL	Turner syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Gonadotrophin pulsatility in girls with the Turner syndrome : modulation by exogenous sex steroids .
	manualset3
85031	4	397999	14	13	NULL	NULL	NULL	 exogenous sex steroids	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gonadotrophin pulsatility in girls with the Turner syndrome : modulation by exogenous sex steroids .
	manualset3
85432	5	397999	14	13	NULL	0	NULL	modulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Gonadotrophin pulsatility in girls with the Turner syndrome : modulation by exogenous sex steroids .
	manualset3
85032	1	398000	14	13	NULL	0	NULL	Gonadotropin-treated ewes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Gonadotropin-treated ewes demonstrated estrus approximately 24 h earlier than control ewes and , therefore , exhibited an accelerated estradiol-17beta surge and rise in circulating progesterone .
	manualset3
85033	2	398000	14	13	NULL	0	NULL	estrus	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gonadotropin-treated ewes demonstrated estrus approximately 24 h earlier than control ewes and , therefore , exhibited an accelerated estradiol-17beta surge and rise in circulating progesterone .
	manualset3
85034	3	398000	14	13	NULL	0	NULL	24 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Gonadotropin-treated ewes demonstrated estrus approximately 24 h earlier than control ewes and , therefore , exhibited an accelerated estradiol-17beta surge and rise in circulating progesterone .
	manualset3
85035	4	398000	14	13	NULL	0	NULL	control ewes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Gonadotropin-treated ewes demonstrated estrus approximately 24 h earlier than control ewes and , therefore , exhibited an accelerated estradiol-17beta surge and rise in circulating progesterone .
	manualset3
85036	5	398000	14	13	NULL	0	NULL	estradiol-17beta surge	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gonadotropin-treated ewes demonstrated estrus approximately 24 h earlier than control ewes and , therefore , exhibited an accelerated estradiol-17beta surge and rise in circulating progesterone .
	manualset3
85037	6	398000	14	13	NULL	0	NULL	rise in circulating progesterone	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gonadotropin-treated ewes demonstrated estrus approximately 24 h earlier than control ewes and , therefore , exhibited an accelerated estradiol-17beta surge and rise in circulating progesterone .
	manualset3
85038	1	398001	14	13	NULL	0	NULL	103 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Good accuracy and recoveries of 103 % were calculated using the fast direct determination technique .
	manualset3
85039	2	398001	14	13	NULL	0	NULL	fast direct determination technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Good accuracy and recoveries of 103 % were calculated using the fast direct determination technique .
	manualset3
85040	1	398002	14	13	NULL	NULL	NULL	 insilico hot spot predictions	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Good agreement between the insilico hot spot predictions and the experimentally observed positions of the polar hydrogen bond forming functional groups and hydrophobic portions was obtained .
	manualset3
85041	2	398002	14	13	NULL	NULL	NULL	experimentally observed positions 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Good agreement between the insilico hot spot predictions and the experimentally observed positions of the polar hydrogen bond forming functional groups and hydrophobic portions was obtained .
	manualset3
85042	3	398002	14	13	NULL	NULL	NULL	 polar hydrogen bond forming functional groups	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Good agreement between the insilico hot spot predictions and the experimentally observed positions of the polar hydrogen bond forming functional groups and hydrophobic portions was obtained .
	manualset3
85436	4	398002	14	13	NULL	0	NULL	hydrophobic portions	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Good agreement between the insilico hot spot predictions and the experimentally observed positions of the polar hydrogen bond forming functional groups and hydrophobic portions was obtained .
	manualset3
85044	1	398003	14	13	NULL	0	NULL	Good birth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Good birth and infertility : a long-awaited homebirth .
	manualset3
85045	2	398003	14	13	NULL	0	NULL	infertility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Good birth and infertility : a long-awaited homebirth .
	manualset3
85046	3	398003	14	13	NULL	0	NULL	 a long-awaited homebirth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Good birth and infertility : a long-awaited homebirth .
	manualset3
85047	1	398004	14	13	NULL	NULL	NULL	Spermatozoal granuloma	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Spermatozoal granuloma as a possible cause of hydrocele ) .
	manualset3
85048	2	398004	14	13	NULL	0	NULL	hydrocele	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Spermatozoal granuloma as a possible cause of hydrocele ) .
	manualset3
85049	1	398005	14	13	NULL	0	NULL	Good communication skills	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Good communication skills and sensitivity are essential to discuss the patient 's needs and preferences and suggest solutions that are safe and legally defensible .
	manualset3
85050	2	398005	14	13	NULL	0	NULL	sensitivity	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Good communication skills and sensitivity are essential to discuss the patient 's needs and preferences and suggest solutions that are safe and legally defensible .
	manualset3
85051	3	398005	14	13	NULL	NULL	NULL	patient 's needs	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Good communication skills and sensitivity are essential to discuss the patient 's needs and preferences and suggest solutions that are safe and legally defensible .
	manualset3
85052	4	398005	14	13	NULL	NULL	NULL	solutions	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Good communication skills and sensitivity are essential to discuss the patient 's needs and preferences and suggest solutions that are safe and legally defensible .
	manualset3
85053	1	398006	14	13	NULL	0	NULL	Good computer	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	Good computer -- bad computer .
	manualset3
85054	2	398006	14	13	NULL	0	NULL	bad computer	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	Good computer -- bad computer .
	manualset3
85055	1	398007	14	13	NULL	NULL	NULL	Good cycle control	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Good cycle control and effective contraception was achieved with the two LNG preparations , however , the cycle control results were less favorable with EE/NET 20/500 .
	manualset3
85056	2	398007	14	13	NULL	NULL	NULL	effective contraception	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Good cycle control and effective contraception was achieved with the two LNG preparations , however , the cycle control results were less favorable with EE/NET 20/500 .
	manualset3
85057	3	398007	14	13	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Good cycle control and effective contraception was achieved with the two LNG preparations , however , the cycle control results were less favorable with EE/NET 20/500 .
	manualset3
85058	4	398007	14	13	NULL	0	NULL	LNG preparations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Good cycle control and effective contraception was achieved with the two LNG preparations , however , the cycle control results were less favorable with EE/NET 20/500 .
	manualset3
85059	5	398007	14	13	NULL	NULL	NULL	cycle control results 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Good cycle control and effective contraception was achieved with the two LNG preparations , however , the cycle control results were less favorable with EE/NET 20/500 .
	manualset3
85060	6	398007	14	13	NULL	0	NULL	EE/NET 20/500	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Good cycle control and effective contraception was achieved with the two LNG preparations , however , the cycle control results were less favorable with EE/NET 20/500 .
	manualset3
85061	1	398008	14	13	NULL	0	NULL	data	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Good precision is obtained when data are acquired for approximately 1 min per sample .
	manualset3
85062	2	398008	14	13	NULL	0	NULL	1 min per sample	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Good precision is obtained when data are acquired for approximately 1 min per sample .
	manualset3
85063	1	398009	14	13	NULL	NULL	NULL	Good recoveries ( 72-129 % )	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Good recoveries ( 72-129 % ) , and low limits of detection ( 0.4-5 .5 ng L ( -1 ) ) and quantification ( 1.1-18 .2 ng L ( -1 ) ) were achieved for all selected pesticides .
	manualset3
85064	2	398009	14	13	NULL	0	NULL	low limits of detection ( 0.4-5 .5 ng L ( -1 ) )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Good recoveries ( 72-129 % ) , and low limits of detection ( 0.4-5 .5 ng L ( -1 ) ) and quantification ( 1.1-18 .2 ng L ( -1 ) ) were achieved for all selected pesticides .
	manualset3
85065	3	398009	14	13	NULL	0	NULL	quantification ( 1.1-18 .2 ng L ( -1 ) )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Good recoveries ( 72-129 % ) , and low limits of detection ( 0.4-5 .5 ng L ( -1 ) ) and quantification ( 1.1-18 .2 ng L ( -1 ) ) were achieved for all selected pesticides .
	manualset3
85066	4	398009	14	13	NULL	0	NULL	all selected pesticides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Good recoveries ( 72-129 % ) , and low limits of detection ( 0.4-5 .5 ng L ( -1 ) ) and quantification ( 1.1-18 .2 ng L ( -1 ) ) were achieved for all selected pesticides .
	manualset3
85067	1	398010	14	13	NULL	0	NULL	Good staining	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Good staining was obtained with ethanol - , glutaraldehyde - , or Carnoy 's - fixed material but not with formalin or Bouin 's fixation .
	manualset3
85068	2	398010	14	13	NULL	NULL	NULL	ethanol -fixed material	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Good staining was obtained with ethanol - , glutaraldehyde - , or Carnoy 's - fixed material but not with formalin or Bouin 's fixation .
	manualset3
85069	3	398010	14	13	NULL	0	NULL	glutaraldehyde -fixed material 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Good staining was obtained with ethanol - , glutaraldehyde - , or Carnoy 's - fixed material but not with formalin or Bouin 's fixation .
	manualset3
85070	4	398010	14	13	NULL	0	NULL	Carnoy 's - fixed material	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Good staining was obtained with ethanol - , glutaraldehyde - , or Carnoy 's - fixed material but not with formalin or Bouin 's fixation .
	manualset3
85071	5	398010	14	13	NULL	0	NULL	formalin fixation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Good staining was obtained with ethanol - , glutaraldehyde - , or Carnoy 's - fixed material but not with formalin or Bouin 's fixation .
	manualset3
85072	6	398010	14	13	NULL	0	NULL	Bouin 's fixation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Good staining was obtained with ethanol - , glutaraldehyde - , or Carnoy 's - fixed material but not with formalin or Bouin 's fixation .
	manualset3
85073	1	398011	14	13	NULL	0	NULL	Goodpasture 's original article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Goodpasture 's original article is reviewed with particular reference to the possible etiological relationship of influenza virus infection and the subsequent development of this strange , poorly understood disorder .
	manualset3
85075	2	398011	14	13	NULL	NULL	NULL	influenza virus infection	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Goodpasture 's original article is reviewed with particular reference to the possible etiological relationship of influenza virus infection and the subsequent development of this strange , poorly understood disorder .
	manualset3
85076	3	398011	14	13	NULL	NULL	NULL	disorder	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Goodpasture 's original article is reviewed with particular reference to the possible etiological relationship of influenza virus infection and the subsequent development of this strange , poorly understood disorder .
	manualset3
85077	1	398012	14	13	NULL	0	NULL	Gout 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Gout in the geriatric patient is a disease affecting women , commonly associated with diuretic usage , often involves the fingers , may be complicated by the development of masses of uric acid crystals ( tophi ) in soft tissues , and is frequently polyarticular .
	manualset3
85078	2	398012	14	13	NULL	0	NULL	geriatric patient	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Gout in the geriatric patient is a disease affecting women , commonly associated with diuretic usage , often involves the fingers , may be complicated by the development of masses of uric acid crystals ( tophi ) in soft tissues , and is frequently polyarticular .
	manualset3
85079	3	398012	14	13	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Gout in the geriatric patient is a disease affecting women , commonly associated with diuretic usage , often involves the fingers , may be complicated by the development of masses of uric acid crystals ( tophi ) in soft tissues , and is frequently polyarticular .
	manualset3
85080	4	398012	14	13	NULL	0	NULL	diuretic usage	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Gout in the geriatric patient is a disease affecting women , commonly associated with diuretic usage , often involves the fingers , may be complicated by the development of masses of uric acid crystals ( tophi ) in soft tissues , and is frequently polyarticular .
	manualset3
85081	5	398012	14	13	NULL	0	NULL	fingers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Gout in the geriatric patient is a disease affecting women , commonly associated with diuretic usage , often involves the fingers , may be complicated by the development of masses of uric acid crystals ( tophi ) in soft tissues , and is frequently polyarticular .
	manualset3
85082	6	398012	14	13	NULL	0	NULL	development of masses of uric acid crystals ( tophi )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gout in the geriatric patient is a disease affecting women , commonly associated with diuretic usage , often involves the fingers , may be complicated by the development of masses of uric acid crystals ( tophi ) in soft tissues , and is frequently polyarticular .
	manualset3
85083	7	398012	14	13	NULL	0	NULL	soft tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Gout in the geriatric patient is a disease affecting women , commonly associated with diuretic usage , often involves the fingers , may be complicated by the development of masses of uric acid crystals ( tophi ) in soft tissues , and is frequently polyarticular .
	manualset3
85084	8	398012	14	13	NULL	0	NULL	polyarticular 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gout in the geriatric patient is a disease affecting women , commonly associated with diuretic usage , often involves the fingers , may be complicated by the development of masses of uric acid crystals ( tophi ) in soft tissues , and is frequently polyarticular .
	manualset3
85085	1	398013	14	13	NULL	0	NULL	Spontaneous rupture of the ureter	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Spontaneous rupture of the ureter caused by metastatic ureteric tumor : a case report ) .
	manualset3
85086	2	398013	14	13	NULL	0	NULL	metastatic ureteric tumor	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Spontaneous rupture of the ureter caused by metastatic ureteric tumor : a case report ) .
	manualset3
85087	3	398013	14	13	NULL	0	NULL	a case report	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Spontaneous rupture of the ureter caused by metastatic ureteric tumor : a case report ) .
	manualset3
85088	1	398014	14	13	NULL	0	NULL	Governmental policy statements	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Governmental policy statements on population : an inventory .
	manualset3
85089	2	398014	14	13	NULL	0	NULL	population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Governmental policy statements on population : an inventory .
	manualset3
85090	1	398015	14	13	NULL	0	NULL	Graded intravenous infusions of vasopressin	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Graded intravenous infusions of vasopressin induced greater increases in MABP and mesenteric vascular resistance and a greater decrease in mesenteric blood flow in males .
	manualset3
85091	2	398015	14	13	NULL	0	NULL	greater increases in MABP	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Graded intravenous infusions of vasopressin induced greater increases in MABP and mesenteric vascular resistance and a greater decrease in mesenteric blood flow in males .
	manualset3
85092	3	398015	14	13	NULL	0	NULL	mesenteric vascular resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Graded intravenous infusions of vasopressin induced greater increases in MABP and mesenteric vascular resistance and a greater decrease in mesenteric blood flow in males .
	manualset3
85093	4	398015	14	13	NULL	0	NULL	greater decrease in mesenteric blood flow	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Graded intravenous infusions of vasopressin induced greater increases in MABP and mesenteric vascular resistance and a greater decrease in mesenteric blood flow in males .
	manualset3
85094	5	398015	14	13	NULL	0	NULL	males	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Graded intravenous infusions of vasopressin induced greater increases in MABP and mesenteric vascular resistance and a greater decrease in mesenteric blood flow in males .
	manualset3
85095	1	398016	14	13	NULL	0	NULL	Graded responsibility and autonomy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Graded responsibility and autonomy are integral features of medical education .
	manualset3
85096	2	398016	14	13	NULL	NULL	NULL	medical education	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Graded responsibility and autonomy are integral features of medical education .
	manualset3
85097	1	398017	14	13	NULL	NULL	NULL	Gradual facial palsy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gradual facial palsy and intrapetrous internal carotid aneurysm : a case report .
	manualset3
85098	2	398017	14	13	NULL	NULL	NULL	intrapetrous internal carotid aneurysm	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gradual facial palsy and intrapetrous internal carotid aneurysm : a case report .
	manualset3
85099	3	398017	14	13	NULL	0	NULL	a case report	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Gradual facial palsy and intrapetrous internal carotid aneurysm : a case report .
	manualset3
85100	1	398018	14	13	NULL	0	NULL	Graft thrombogenicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Graft thrombogenicity was assessed by changes in platelet function , isotope labeled platelet studies and scanning electron microscopy .
	manualset3
85101	2	398018	14	13	NULL	NULL	NULL	changes in platelet function	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Graft thrombogenicity was assessed by changes in platelet function , isotope labeled platelet studies and scanning electron microscopy .
	manualset3
85102	3	398018	14	13	NULL	0	NULL	isotope labeled platelet studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Graft thrombogenicity was assessed by changes in platelet function , isotope labeled platelet studies and scanning electron microscopy .
	manualset3
85103	4	398018	14	13	NULL	0	NULL	 scanning electron microscopy	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Graft thrombogenicity was assessed by changes in platelet function , isotope labeled platelet studies and scanning electron microscopy .
	manualset3
85104	1	398019	14	13	NULL	0	NULL	Graft versus host disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Graft versus host disease-dependent decreases in salivary IgA levels were sought in labial gland saliva samples from bone marrow transplant recipients .
	manualset3
85105	2	398019	14	13	NULL	0	NULL	salivary IgA levels	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Graft versus host disease-dependent decreases in salivary IgA levels were sought in labial gland saliva samples from bone marrow transplant recipients .
	manualset3
85106	3	398019	14	13	NULL	0	NULL	labial gland saliva samples	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Graft versus host disease-dependent decreases in salivary IgA levels were sought in labial gland saliva samples from bone marrow transplant recipients .
	manualset3
85107	4	398019	14	13	NULL	0	NULL	bone marrow transplant recipients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Graft versus host disease-dependent decreases in salivary IgA levels were sought in labial gland saliva samples from bone marrow transplant recipients .
	manualset3
85108	1	398020	14	13	NULL	0	NULL	Graft versus host disease ( GVHD ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Graft versus host disease ( GVHD ) is one of the obstacles encountered in allogeneic bone marrow transplantation ( alloBMT ) and has a direct impact on the transplant outcome and survival .
	manualset3
85109	2	398020	14	13	NULL	0	NULL	allogeneic bone marrow transplantation ( alloBMT ) 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Graft versus host disease ( GVHD ) is one of the obstacles encountered in allogeneic bone marrow transplantation ( alloBMT ) and has a direct impact on the transplant outcome and survival .
	manualset3
85110	3	398020	14	13	NULL	0	NULL	 transplant outcome and survival 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Graft versus host disease ( GVHD ) is one of the obstacles encountered in allogeneic bone marrow transplantation ( alloBMT ) and has a direct impact on the transplant outcome and survival .
	manualset3
85111	1	398021	14	13	NULL	0	NULL	Gram-positive bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Gram-positive bacteria and fungus accounted for 22.1 % ( 25/113 ) and 21.2 % ( 24/113 ) of the isolated strains , respectively .
	manualset3
85112	2	398021	14	13	NULL	NULL	NULL	fungus	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gram-positive bacteria and fungus accounted for 22.1 % ( 25/113 ) and 21.2 % ( 24/113 ) of the isolated strains , respectively .
	manualset3
85113	3	398021	14	13	NULL	0	NULL	22.1 % ( 25/113 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Gram-positive bacteria and fungus accounted for 22.1 % ( 25/113 ) and 21.2 % ( 24/113 ) of the isolated strains , respectively .
	manualset3
85114	4	398021	14	13	NULL	0	NULL	21.2 % ( 24/113 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Gram-positive bacteria and fungus accounted for 22.1 % ( 25/113 ) and 21.2 % ( 24/113 ) of the isolated strains , respectively .
	manualset3
85115	5	398021	14	13	NULL	0	NULL	isolated strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Gram-positive bacteria and fungus accounted for 22.1 % ( 25/113 ) and 21.2 % ( 24/113 ) of the isolated strains , respectively .
	manualset3
85116	1	398022	14	13	NULL	0	NULL	Gram-positive bloodstream infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gram-positive bloodstream infections in liver transplant recipients : incidence , risk factors , and impact on survival .
	manualset3
85117	2	398022	14	13	NULL	0	NULL	liver transplant recipients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Gram-positive bloodstream infections in liver transplant recipients : incidence , risk factors , and impact on survival .
	manualset3
85118	3	398022	14	13	NULL	0	NULL	 incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gram-positive bloodstream infections in liver transplant recipients : incidence , risk factors , and impact on survival .
	manualset3
85119	4	398022	14	13	NULL	0	NULL	risk factors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gram-positive bloodstream infections in liver transplant recipients : incidence , risk factors , and impact on survival .
	manualset3
85120	5	398022	14	13	NULL	0	NULL	impact on survival 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gram-positive bloodstream infections in liver transplant recipients : incidence , risk factors , and impact on survival .
	manualset3
85121	1	398023	14	13	NULL	0	NULL	Gram negative diplococci 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Gram negative diplococci grown on selective media and which are catalase , oxidase , DNase , nitrate reduction positive , glucose , maltose , sucrose and lactose fermentation negative , were diagnosed as M. catarrhalis .
	manualset3
85122	3	398023	14	13	NULL	NULL	NULL	catalase	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gram negative diplococci grown on selective media and which are catalase , oxidase , DNase , nitrate reduction positive , glucose , maltose , sucrose and lactose fermentation negative , were diagnosed as M. catarrhalis .
	manualset3
85124	4	398023	14	13	NULL	NULL	NULL	oxidase	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gram negative diplococci grown on selective media and which are catalase , oxidase , DNase , nitrate reduction positive , glucose , maltose , sucrose and lactose fermentation negative , were diagnosed as M. catarrhalis .
	manualset3
85126	2	398023	14	13	NULL	NULL	NULL	DNase	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gram negative diplococci grown on selective media and which are catalase , oxidase , DNase , nitrate reduction positive , glucose , maltose , sucrose and lactose fermentation negative , were diagnosed as M. catarrhalis .
	manualset3
85127	5	398023	14	13	NULL	NULL	NULL	nitrate	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gram negative diplococci grown on selective media and which are catalase , oxidase , DNase , nitrate reduction positive , glucose , maltose , sucrose and lactose fermentation negative , were diagnosed as M. catarrhalis .
	manualset3
85128	6	398023	14	13	NULL	NULL	NULL	glucose 	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gram negative diplococci grown on selective media and which are catalase , oxidase , DNase , nitrate reduction positive , glucose , maltose , sucrose and lactose fermentation negative , were diagnosed as M. catarrhalis .
	manualset3
85129	7	398023	14	13	NULL	NULL	NULL	maltose	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gram negative diplococci grown on selective media and which are catalase , oxidase , DNase , nitrate reduction positive , glucose , maltose , sucrose and lactose fermentation negative , were diagnosed as M. catarrhalis .
	manualset3
85130	8	398023	14	13	NULL	NULL	NULL	sucrose	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gram negative diplococci grown on selective media and which are catalase , oxidase , DNase , nitrate reduction positive , glucose , maltose , sucrose and lactose fermentation negative , were diagnosed as M. catarrhalis .
	manualset3
85131	9	398023	14	13	NULL	NULL	NULL	lactose	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gram negative diplococci grown on selective media and which are catalase , oxidase , DNase , nitrate reduction positive , glucose , maltose , sucrose and lactose fermentation negative , were diagnosed as M. catarrhalis .
	manualset3
85132	10	398023	14	13	NULL	0	NULL	M. catarrhalis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Gram negative diplococci grown on selective media and which are catalase , oxidase , DNase , nitrate reduction positive , glucose , maltose , sucrose and lactose fermentation negative , were diagnosed as M. catarrhalis .
	manualset3
85133	1	398024	14	13	NULL	0	NULL	 Spread of excitation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Spread of excitation from the ventromedial hypothalamus to the limbic-reticular structure of the brain ) .
	manualset3
85134	2	398024	14	13	NULL	0	NULL	ventromedial hypothalamus	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Spread of excitation from the ventromedial hypothalamus to the limbic-reticular structure of the brain ) .
	manualset3
85135	3	398024	14	13	NULL	0	NULL	limbic-reticular structure of the brain	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Spread of excitation from the ventromedial hypothalamus to the limbic-reticular structure of the brain ) .
	manualset3
85136	1	398025	14	13	NULL	0	NULL	Grammar	Language												NULL		0	NULL	NULL	NULL	NULL	NULL	Grammar and syntax for UVAL-MED are defined and its features as a language-independent tool are discussed .
	manualset3
85137	2	398025	14	13	NULL	0	NULL	syntax	Language												NULL		0	NULL	NULL	NULL	NULL	NULL	Grammar and syntax for UVAL-MED are defined and its features as a language-independent tool are discussed .
	manualset3
85138	3	398025	14	13	NULL	0	NULL	UVAL-MED	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Grammar and syntax for UVAL-MED are defined and its features as a language-independent tool are discussed .
	manualset3
85139	4	398025	14	13	NULL	0	NULL	language-independent tool	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Grammar and syntax for UVAL-MED are defined and its features as a language-independent tool are discussed .
	manualset3
85140	1	398026	14	13	NULL	0	NULL	Granular acute lymphoblastic leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Granular acute lymphoblastic leukemia in an adult patient .
	manualset3
85141	2	398026	14	13	NULL	NULL	NULL	adult patient	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Granular acute lymphoblastic leukemia in an adult patient .
	manualset3
85142	1	398027	14	13	NULL	0	NULL	Granulocyte antibodies	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Granulocyte antibodies are important in the pathogenesis of neonatal granulocytopenia , in some varieties of idiopathic granulocytopenia , and in transfusion reactions , particularly since the development of leukocyte transfusion therapy for granulocytopenic patients .
	manualset3
85143	2	398027	14	13	NULL	0	NULL	pathogenesis of neonatal granulocytopenia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Granulocyte antibodies are important in the pathogenesis of neonatal granulocytopenia , in some varieties of idiopathic granulocytopenia , and in transfusion reactions , particularly since the development of leukocyte transfusion therapy for granulocytopenic patients .
	manualset3
85144	3	398027	14	13	NULL	NULL	NULL	idiopathic granulocytopenia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Granulocyte antibodies are important in the pathogenesis of neonatal granulocytopenia , in some varieties of idiopathic granulocytopenia , and in transfusion reactions , particularly since the development of leukocyte transfusion therapy for granulocytopenic patients .
	manualset3
85145	4	398027	14	13	NULL	NULL	NULL	 transfusion reactions 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Granulocyte antibodies are important in the pathogenesis of neonatal granulocytopenia , in some varieties of idiopathic granulocytopenia , and in transfusion reactions , particularly since the development of leukocyte transfusion therapy for granulocytopenic patients .
	manualset3
85146	5	398027	14	13	NULL	NULL	NULL	leukocyte transfusion therapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Granulocyte antibodies are important in the pathogenesis of neonatal granulocytopenia , in some varieties of idiopathic granulocytopenia , and in transfusion reactions , particularly since the development of leukocyte transfusion therapy for granulocytopenic patients .
	manualset3
85147	6	398027	14	13	NULL	0	NULL	granulocytopenic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Granulocyte antibodies are important in the pathogenesis of neonatal granulocytopenia , in some varieties of idiopathic granulocytopenia , and in transfusion reactions , particularly since the development of leukocyte transfusion therapy for granulocytopenic patients .
	manualset3
85148	1	398028	14	13	NULL	0	NULL	Granulocyte macrophage colony-stimulating factor ( GM-CSF )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Granulocyte macrophage colony-stimulating factor ( GM-CSF ) has been shown to be an effective vaccine adjuvant because it enhances antigen processing and presentation by dendritic cells .
	manualset3
85149	2	398028	14	13	NULL	0	NULL	effective vaccine adjuvant	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Granulocyte macrophage colony-stimulating factor ( GM-CSF ) has been shown to be an effective vaccine adjuvant because it enhances antigen processing and presentation by dendritic cells .
	manualset3
85150	3	398028	14	13	NULL	0	NULL	antigen processing and presentation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Granulocyte macrophage colony-stimulating factor ( GM-CSF ) has been shown to be an effective vaccine adjuvant because it enhances antigen processing and presentation by dendritic cells .
	manualset3
85151	4	398028	14	13	NULL	0	NULL	dendritic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Granulocyte macrophage colony-stimulating factor ( GM-CSF ) has been shown to be an effective vaccine adjuvant because it enhances antigen processing and presentation by dendritic cells .
	manualset3
85152	1	398029	14	13	NULL	0	NULL	Granulocytic sarcoma ( chloroma )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Granulocytic sarcoma ( chloroma ) is a rare solid tumor of myelogenous stem cells , usually appearing in patients with acute myelogenous leukemia and less commonly in patients with chronic myelogenous leukemia or myeloproliferative disorders .
	manualset3
85153	2	398029	14	13	NULL	NULL	NULL	rare solid tumor	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Granulocytic sarcoma ( chloroma ) is a rare solid tumor of myelogenous stem cells , usually appearing in patients with acute myelogenous leukemia and less commonly in patients with chronic myelogenous leukemia or myeloproliferative disorders .
	manualset3
85154	3	398029	14	13	NULL	0	NULL	myelogenous stem cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Granulocytic sarcoma ( chloroma ) is a rare solid tumor of myelogenous stem cells , usually appearing in patients with acute myelogenous leukemia and less commonly in patients with chronic myelogenous leukemia or myeloproliferative disorders .
	manualset3
85155	4	398029	14	13	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Granulocytic sarcoma ( chloroma ) is a rare solid tumor of myelogenous stem cells , usually appearing in patients with acute myelogenous leukemia and less commonly in patients with chronic myelogenous leukemia or myeloproliferative disorders .
	manualset3
85156	5	398029	14	13	NULL	0	NULL	acute myelogenous leukemia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Granulocytic sarcoma ( chloroma ) is a rare solid tumor of myelogenous stem cells , usually appearing in patients with acute myelogenous leukemia and less commonly in patients with chronic myelogenous leukemia or myeloproliferative disorders .
	manualset3
85157	6	398029	14	13	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Granulocytic sarcoma ( chloroma ) is a rare solid tumor of myelogenous stem cells , usually appearing in patients with acute myelogenous leukemia and less commonly in patients with chronic myelogenous leukemia or myeloproliferative disorders .
	manualset3
85158	7	398029	14	13	NULL	0	NULL	chronic myelogenous leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Granulocytic sarcoma ( chloroma ) is a rare solid tumor of myelogenous stem cells , usually appearing in patients with acute myelogenous leukemia and less commonly in patients with chronic myelogenous leukemia or myeloproliferative disorders .
	manualset3
85159	8	398029	14	13	NULL	0	NULL	myeloproliferative disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Granulocytic sarcoma ( chloroma ) is a rare solid tumor of myelogenous stem cells , usually appearing in patients with acute myelogenous leukemia and less commonly in patients with chronic myelogenous leukemia or myeloproliferative disorders .
	manualset3
85160	1	398030	14	13	NULL	0	NULL	Granulocytic sarcoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Granulocytic sarcoma of the testis .
	manualset3
85161	2	398030	14	13	NULL	0	NULL	testis 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Granulocytic sarcoma of the testis .
	manualset3
83290	1	398031	5	NULL	NULL	0	NULL	Graves ' disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Graves ' disease also resolved but without specific treatment with either antithyroid drugs or radioactive iodine .
	manualset3
83291	2	398031	5	NULL	NULL	0	NULL	specific treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Graves ' disease also resolved but without specific treatment with either antithyroid drugs or radioactive iodine .
	manualset3
83292	3	398031	5	NULL	NULL	0	NULL	antithyroid drugs	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Graves ' disease also resolved but without specific treatment with either antithyroid drugs or radioactive iodine .
	manualset3
83293	4	398031	5	NULL	NULL	0	NULL	radioactive iodine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Graves ' disease also resolved but without specific treatment with either antithyroid drugs or radioactive iodine .
	manualset3
83294	1	398032	5	NULL	NULL	0	NULL	time savings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Greater autonomy and time savings ) .
	manualset3
83295	1	398033	5	NULL	NULL	0	NULL	young	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Greater opportunities for the young and women in socioeconomic areas will tend to increase participation in decisions which will moderate fertility .
	manualset3
83296	2	398033	5	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Greater opportunities for the young and women in socioeconomic areas will tend to increase participation in decisions which will moderate fertility .
	manualset3
83297	3	398033	5	NULL	NULL	0	NULL	socioeconomic areas	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Greater opportunities for the young and women in socioeconomic areas will tend to increase participation in decisions which will moderate fertility .
	manualset3
83298	4	398033	5	NULL	NULL	0	NULL	increase participation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Greater opportunities for the young and women in socioeconomic areas will tend to increase participation in decisions which will moderate fertility .
	manualset3
83299	5	398033	5	NULL	NULL	0	NULL	decisions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Greater opportunities for the young and women in socioeconomic areas will tend to increase participation in decisions which will moderate fertility .
	manualset3
83300	6	398033	5	NULL	NULL	0	NULL	moderate fertility	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Greater opportunities for the young and women in socioeconomic areas will tend to increase participation in decisions which will moderate fertility .
	manualset3
83301	1	398034	5	NULL	NULL	0	NULL	Greater attention	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Greater attention has been focused on the criteria for listing patients for transplantation and for allocation of organs .
	manualset3
83302	2	398034	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Greater attention has been focused on the criteria for listing patients for transplantation and for allocation of organs .
	manualset3
83303	3	398034	5	NULL	NULL	NULL	NULL	transplantation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Greater attention has been focused on the criteria for listing patients for transplantation and for allocation of organs .
	manualset3
83304	4	398034	5	NULL	NULL	0	NULL	allocation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Greater attention has been focused on the criteria for listing patients for transplantation and for allocation of organs .
	manualset3
83305	5	398034	5	NULL	NULL	0	NULL	organs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Greater attention has been focused on the criteria for listing patients for transplantation and for allocation of organs .
	manualset3
83306	1	398035	5	NULL	NULL	0	NULL	Green sulfur bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Green sulfur bacteria utilize reduced inorganic sulfur compounds ( sulfide , thiosulfate , and/or sulfur ) as electron sources for their anoxygenic photosynthetic growth .
	manualset3
83307	2	398035	5	NULL	NULL	0	NULL	reduced inorganic sulfur compounds ( sulfide , thiosulfate , and/or sulfur )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Green sulfur bacteria utilize reduced inorganic sulfur compounds ( sulfide , thiosulfate , and/or sulfur ) as electron sources for their anoxygenic photosynthetic growth .
	manualset3
83308	3	398035	5	NULL	NULL	0	NULL	electron sources	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Green sulfur bacteria utilize reduced inorganic sulfur compounds ( sulfide , thiosulfate , and/or sulfur ) as electron sources for their anoxygenic photosynthetic growth .
	manualset3
83309	4	398035	5	NULL	NULL	0	NULL	anoxygenic photosynthetic growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Green sulfur bacteria utilize reduced inorganic sulfur compounds ( sulfide , thiosulfate , and/or sulfur ) as electron sources for their anoxygenic photosynthetic growth .
	manualset3
83310	1	398036	5	NULL	NULL	0	NULL	Green tea consumption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Green tea consumption tended to reduce aortic lesion formation by 31 % ( 24 + / - 3.2 % versus 35 + / - 5.7 % for control animals P = 0.11 ) , while black tea , vitamin E and beta-carotene had no effect .
	manualset3
83311	2	398036	5	NULL	NULL	0	NULL	reduce aortic lesion formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Green tea consumption tended to reduce aortic lesion formation by 31 % ( 24 + / - 3.2 % versus 35 + / - 5.7 % for control animals P = 0.11 ) , while black tea , vitamin E and beta-carotene had no effect .
	manualset3
83312	3	398036	5	NULL	NULL	0	NULL	31 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Green tea consumption tended to reduce aortic lesion formation by 31 % ( 24 + / - 3.2 % versus 35 + / - 5.7 % for control animals P = 0.11 ) , while black tea , vitamin E and beta-carotene had no effect .
	manualset3
83313	4	398036	5	NULL	NULL	0	NULL	( 24 + / - 3.2 % versus 35 + / - 5.7 % for control animals P = 0.11 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Green tea consumption tended to reduce aortic lesion formation by 31 % ( 24 + / - 3.2 % versus 35 + / - 5.7 % for control animals P = 0.11 ) , while black tea , vitamin E and beta-carotene had no effect .
	manualset3
83314	5	398036	5	NULL	NULL	0	NULL	black tea	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Green tea consumption tended to reduce aortic lesion formation by 31 % ( 24 + / - 3.2 % versus 35 + / - 5.7 % for control animals P = 0.11 ) , while black tea , vitamin E and beta-carotene had no effect .
	manualset3
83315	6	398036	5	NULL	NULL	0	NULL	vitamin E	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Green tea consumption tended to reduce aortic lesion formation by 31 % ( 24 + / - 3.2 % versus 35 + / - 5.7 % for control animals P = 0.11 ) , while black tea , vitamin E and beta-carotene had no effect .
	manualset3
83316	7	398036	5	NULL	NULL	0	NULL	beta-carotene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Green tea consumption tended to reduce aortic lesion formation by 31 % ( 24 + / - 3.2 % versus 35 + / - 5.7 % for control animals P = 0.11 ) , while black tea , vitamin E and beta-carotene had no effect .
	manualset3
83317	1	398037	5	NULL	NULL	NULL	NULL	Green tea ( Camellia sinensis )	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Green tea ( Camellia sinensis ) is rich in catechins , of which ( - ) - epigallocatechin-3-gallate ( EGCG ) is the most abundant .
	manualset3
83319	2	398037	5	NULL	NULL	NULL	NULL	catechins	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Green tea ( Camellia sinensis ) is rich in catechins , of which ( - ) - epigallocatechin-3-gallate ( EGCG ) is the most abundant .
	manualset3
83320	3	398037	5	NULL	NULL	NULL	NULL	 ( - ) - epigallocatechin-3-gallate ( EGCG )	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Green tea ( Camellia sinensis ) is rich in catechins , of which ( - ) - epigallocatechin-3-gallate ( EGCG ) is the most abundant .
	manualset3
83321	1	398038	5	NULL	NULL	0	NULL	Green space	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Green space , health inequality and pregnancy .
	manualset3
83322	2	398038	5	NULL	NULL	0	NULL	health inequality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Green space , health inequality and pregnancy .
	manualset3
83323	3	398038	5	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Green space , health inequality and pregnancy .
	manualset3
83324	1	398039	5	NULL	NULL	0	NULL	Gregory Bisson	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Gregory Bisson and Jeffrey Stringer discuss the implications of a new study showing how loss to follow-up affects the effectiveness of a public sector HIV program in Cte d'Ivoire .
	manualset3
83325	2	398039	5	NULL	NULL	0	NULL	Jeffrey Stringer	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Gregory Bisson and Jeffrey Stringer discuss the implications of a new study showing how loss to follow-up affects the effectiveness of a public sector HIV program in Cte d'Ivoire .
	manualset3
83326	3	398039	5	NULL	NULL	0	NULL	implications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Gregory Bisson and Jeffrey Stringer discuss the implications of a new study showing how loss to follow-up affects the effectiveness of a public sector HIV program in Cte d'Ivoire .
	manualset3
83327	4	398039	5	NULL	NULL	0	NULL	new study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Gregory Bisson and Jeffrey Stringer discuss the implications of a new study showing how loss to follow-up affects the effectiveness of a public sector HIV program in Cte d'Ivoire .
	manualset3
83328	5	398039	5	NULL	NULL	0	NULL	follow-up	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Gregory Bisson and Jeffrey Stringer discuss the implications of a new study showing how loss to follow-up affects the effectiveness of a public sector HIV program in Cte d'Ivoire .
	manualset3
83329	6	398039	5	NULL	NULL	0	NULL	public sector HIV program	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Gregory Bisson and Jeffrey Stringer discuss the implications of a new study showing how loss to follow-up affects the effectiveness of a public sector HIV program in Cte d'Ivoire .
	manualset3
83330	7	398039	5	NULL	NULL	0	NULL	Cte d'Ivoire	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Gregory Bisson and Jeffrey Stringer discuss the implications of a new study showing how loss to follow-up affects the effectiveness of a public sector HIV program in Cte d'Ivoire .
	manualset3
83331	1	398040	5	NULL	NULL	0	NULL	Grimelius reactivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Grimelius reactivity was identical to chromogranin immunoreactivity in all cases except that more cells in the tumors and in the normal islets were positive for chromogranin .
	manualset3
83332	2	398040	5	NULL	NULL	0	NULL	chromogranin immunoreactivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Grimelius reactivity was identical to chromogranin immunoreactivity in all cases except that more cells in the tumors and in the normal islets were positive for chromogranin .
	manualset3
83333	3	398040	5	NULL	NULL	0	NULL	more cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Grimelius reactivity was identical to chromogranin immunoreactivity in all cases except that more cells in the tumors and in the normal islets were positive for chromogranin .
	manualset3
83334	4	398040	5	NULL	NULL	0	NULL	tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Grimelius reactivity was identical to chromogranin immunoreactivity in all cases except that more cells in the tumors and in the normal islets were positive for chromogranin .
	manualset3
83335	5	398040	5	NULL	NULL	0	NULL	normal islets	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Grimelius reactivity was identical to chromogranin immunoreactivity in all cases except that more cells in the tumors and in the normal islets were positive for chromogranin .
	manualset3
83336	6	398040	5	NULL	NULL	0	NULL	chromogranin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Grimelius reactivity was identical to chromogranin immunoreactivity in all cases except that more cells in the tumors and in the normal islets were positive for chromogranin .
	manualset3
83338	1	398041	5	NULL	NULL	NULL	NULL	occlusion	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( State of the art : posture and occlusion ) .
	manualset3
83339	1	398042	5	NULL	NULL	0	NULL	Ground beef products	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Ground beef products are susceptible to contamination with Escherichia coli O157 : H7 .
	manualset3
83340	2	398042	5	NULL	NULL	0	NULL	contamination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ground beef products are susceptible to contamination with Escherichia coli O157 : H7 .
	manualset3
83341	3	398042	5	NULL	NULL	0	NULL	Escherichia coli O157 : H7	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ground beef products are susceptible to contamination with Escherichia coli O157 : H7 .
	manualset3
83342	1	398043	5	NULL	NULL	NULL	NULL	Ground glass opacification	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ground glass opacification was present in seven , while basal honey-combing was also evident in seven patients .
	manualset3
83343	2	398043	5	NULL	NULL	0	NULL	seven	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ground glass opacification was present in seven , while basal honey-combing was also evident in seven patients .
	manualset3
83344	3	398043	5	NULL	NULL	0	NULL	basal honey-combing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ground glass opacification was present in seven , while basal honey-combing was also evident in seven patients .
	manualset3
83345	4	398043	5	NULL	NULL	0	NULL	seven patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ground glass opacification was present in seven , while basal honey-combing was also evident in seven patients .
	manualset3
83346	1	398044	5	NULL	NULL	0	NULL	Groundwater	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Groundwater contaminated with arsenic must be treated to meet stringent drinking water standards or guideline values .
	manualset3
83347	2	398044	5	NULL	NULL	0	NULL	arsenic	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Groundwater contaminated with arsenic must be treated to meet stringent drinking water standards or guideline values .
	manualset3
83348	3	398044	5	NULL	NULL	0	NULL	stringent drinking water standards	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Groundwater contaminated with arsenic must be treated to meet stringent drinking water standards or guideline values .
	manualset3
83349	4	398044	5	NULL	NULL	0	NULL	guideline values	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Groundwater contaminated with arsenic must be treated to meet stringent drinking water standards or guideline values .
	manualset3
83350	1	398045	5	NULL	NULL	0	NULL	Group 2 and group 3 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 2 and group 3 patients had higher fasting intragastric bile acid concentrations than group 1 ( p less than 0.01 in both cases ) .
	manualset3
83351	2	398045	5	NULL	NULL	0	NULL	higher fasting intragastric bile acid concentrations	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 2 and group 3 patients had higher fasting intragastric bile acid concentrations than group 1 ( p less than 0.01 in both cases ) .
	manualset3
83352	3	398045	5	NULL	NULL	0	NULL	group 1	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 2 and group 3 patients had higher fasting intragastric bile acid concentrations than group 1 ( p less than 0.01 in both cases ) .
	manualset3
83353	4	398045	5	NULL	NULL	0	NULL	 p less than 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 2 and group 3 patients had higher fasting intragastric bile acid concentrations than group 1 ( p less than 0.01 in both cases ) .
	manualset3
83354	1	398046	5	NULL	NULL	0	NULL	Group 3 cats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 3 cats demonstrated the highest detectable antibody response to the vaccine antigen as determined by ELISA and Western blot analysis .
	manualset3
83355	2	398046	5	NULL	NULL	0	NULL	highest detectable antibody response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 3 cats demonstrated the highest detectable antibody response to the vaccine antigen as determined by ELISA and Western blot analysis .
	manualset3
83356	3	398046	5	NULL	NULL	0	NULL	vaccine antigen	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 3 cats demonstrated the highest detectable antibody response to the vaccine antigen as determined by ELISA and Western blot analysis .
	manualset3
83357	4	398046	5	NULL	NULL	0	NULL	ELISA 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 3 cats demonstrated the highest detectable antibody response to the vaccine antigen as determined by ELISA and Western blot analysis .
	manualset3
83358	5	398046	5	NULL	NULL	0	NULL	Western blot analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 3 cats demonstrated the highest detectable antibody response to the vaccine antigen as determined by ELISA and Western blot analysis .
	manualset3
83359	1	398047	5	NULL	NULL	0	NULL	mouth cavity	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( State of the mouth cavity in patients with inflammatory intestinal diseases ) .
	manualset3
83360	2	398047	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( State of the mouth cavity in patients with inflammatory intestinal diseases ) .
	manualset3
83361	3	398047	5	NULL	NULL	0	NULL	inflammatory intestinal diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( State of the mouth cavity in patients with inflammatory intestinal diseases ) .
	manualset3
83362	1	398048	5	NULL	NULL	0	NULL	Group B animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Group B animals also had improved thymic function as assessed by thymic weight , the total number of thymic lymphocytes/gland and mitogenic reactivity of thymic lymphocytes to PHA and Con A. The experiments indicate that high arginine levels in IVH solutions improve wound healing and thymic immune function following injury .
	manualset3
83363	2	398048	5	NULL	NULL	0	NULL	improved thymic function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Group B animals also had improved thymic function as assessed by thymic weight , the total number of thymic lymphocytes/gland and mitogenic reactivity of thymic lymphocytes to PHA and Con A. The experiments indicate that high arginine levels in IVH solutions improve wound healing and thymic immune function following injury .
	manualset3
83364	3	398048	5	NULL	NULL	NULL	NULL	thymic weight	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Group B animals also had improved thymic function as assessed by thymic weight , the total number of thymic lymphocytes/gland and mitogenic reactivity of thymic lymphocytes to PHA and Con A. The experiments indicate that high arginine levels in IVH solutions improve wound healing and thymic immune function following injury .
	manualset3
83365	4	398048	5	NULL	NULL	0	NULL	total number of thymic lymphocytes/gland	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Group B animals also had improved thymic function as assessed by thymic weight , the total number of thymic lymphocytes/gland and mitogenic reactivity of thymic lymphocytes to PHA and Con A. The experiments indicate that high arginine levels in IVH solutions improve wound healing and thymic immune function following injury .
	manualset3
83366	5	398048	5	NULL	NULL	0	NULL	mitogenic reactivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Group B animals also had improved thymic function as assessed by thymic weight , the total number of thymic lymphocytes/gland and mitogenic reactivity of thymic lymphocytes to PHA and Con A. The experiments indicate that high arginine levels in IVH solutions improve wound healing and thymic immune function following injury .
	manualset3
83367	6	398048	5	NULL	NULL	0	NULL	thymic lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Group B animals also had improved thymic function as assessed by thymic weight , the total number of thymic lymphocytes/gland and mitogenic reactivity of thymic lymphocytes to PHA and Con A. The experiments indicate that high arginine levels in IVH solutions improve wound healing and thymic immune function following injury .
	manualset3
83368	7	398048	5	NULL	NULL	0	NULL	PHA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Group B animals also had improved thymic function as assessed by thymic weight , the total number of thymic lymphocytes/gland and mitogenic reactivity of thymic lymphocytes to PHA and Con A. The experiments indicate that high arginine levels in IVH solutions improve wound healing and thymic immune function following injury .
	manualset3
83369	8	398048	5	NULL	NULL	0	NULL	Con A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Group B animals also had improved thymic function as assessed by thymic weight , the total number of thymic lymphocytes/gland and mitogenic reactivity of thymic lymphocytes to PHA and Con A. The experiments indicate that high arginine levels in IVH solutions improve wound healing and thymic immune function following injury .
	manualset3
83370	9	398048	5	NULL	NULL	0	NULL	experiments 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Group B animals also had improved thymic function as assessed by thymic weight , the total number of thymic lymphocytes/gland and mitogenic reactivity of thymic lymphocytes to PHA and Con A. The experiments indicate that high arginine levels in IVH solutions improve wound healing and thymic immune function following injury .
	manualset3
83371	10	398048	5	NULL	NULL	0	NULL	high arginine levels	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Group B animals also had improved thymic function as assessed by thymic weight , the total number of thymic lymphocytes/gland and mitogenic reactivity of thymic lymphocytes to PHA and Con A. The experiments indicate that high arginine levels in IVH solutions improve wound healing and thymic immune function following injury .
	manualset3
83372	11	398048	5	NULL	NULL	0	NULL	IVH solutions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Group B animals also had improved thymic function as assessed by thymic weight , the total number of thymic lymphocytes/gland and mitogenic reactivity of thymic lymphocytes to PHA and Con A. The experiments indicate that high arginine levels in IVH solutions improve wound healing and thymic immune function following injury .
	manualset3
83373	12	398048	5	NULL	NULL	0	NULL	improve wound healing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Group B animals also had improved thymic function as assessed by thymic weight , the total number of thymic lymphocytes/gland and mitogenic reactivity of thymic lymphocytes to PHA and Con A. The experiments indicate that high arginine levels in IVH solutions improve wound healing and thymic immune function following injury .
	manualset3
83374	13	398048	5	NULL	NULL	0	NULL	thymic immune function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Group B animals also had improved thymic function as assessed by thymic weight , the total number of thymic lymphocytes/gland and mitogenic reactivity of thymic lymphocytes to PHA and Con A. The experiments indicate that high arginine levels in IVH solutions improve wound healing and thymic immune function following injury .
	manualset3
83375	14	398048	5	NULL	NULL	0	NULL	injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Group B animals also had improved thymic function as assessed by thymic weight , the total number of thymic lymphocytes/gland and mitogenic reactivity of thymic lymphocytes to PHA and Con A. The experiments indicate that high arginine levels in IVH solutions improve wound healing and thymic immune function following injury .
	manualset3
83376	1	398049	5	NULL	NULL	0	NULL	Group II ( postincisional group ) 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Group II ( postincisional group ) received the same drug mixture after surgery .
	manualset3
83377	2	398049	5	NULL	NULL	0	NULL	drug mixture	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Group II ( postincisional group ) received the same drug mixture after surgery .
	manualset3
83378	3	398049	5	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Group II ( postincisional group ) received the same drug mixture after surgery .
	manualset3
83379	1	398050	5	NULL	NULL	NULL	NULL	Group differences	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Group differences are analyzed through a cultural lens in which different interpretive norms can generate expectations for either nondirectiveness or directiveness .
	manualset3
83380	2	398050	5	NULL	NULL	NULL	NULL	cultural lens	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Group differences are analyzed through a cultural lens in which different interpretive norms can generate expectations for either nondirectiveness or directiveness .
	manualset3
83381	3	398050	5	NULL	NULL	NULL	NULL	different interpretive norms 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Group differences are analyzed through a cultural lens in which different interpretive norms can generate expectations for either nondirectiveness or directiveness .
	manualset3
83382	1	398051	5	NULL	NULL	0	NULL	Groups 3-6 rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Groups 3-6 rats were given DMH at a dose of ( 20mg/kg body weight subcutaneously ) once a week for 15 weeks to induce colonic tumors .
	manualset3
83383	2	398051	5	NULL	NULL	0	NULL	DMH 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Groups 3-6 rats were given DMH at a dose of ( 20mg/kg body weight subcutaneously ) once a week for 15 weeks to induce colonic tumors .
	manualset3
83384	3	398051	5	NULL	NULL	NULL	NULL	dose	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Groups 3-6 rats were given DMH at a dose of ( 20mg/kg body weight subcutaneously ) once a week for 15 weeks to induce colonic tumors .
	manualset3
83385	4	398051	5	NULL	NULL	0	NULL	20mg/kg body weight	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Groups 3-6 rats were given DMH at a dose of ( 20mg/kg body weight subcutaneously ) once a week for 15 weeks to induce colonic tumors .
	manualset3
83386	5	398051	5	NULL	NULL	0	NULL	once a week	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Groups 3-6 rats were given DMH at a dose of ( 20mg/kg body weight subcutaneously ) once a week for 15 weeks to induce colonic tumors .
	manualset3
83387	6	398051	5	NULL	NULL	NULL	NULL	15 weeks	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Groups 3-6 rats were given DMH at a dose of ( 20mg/kg body weight subcutaneously ) once a week for 15 weeks to induce colonic tumors .
	manualset3
83388	7	398051	5	NULL	NULL	0	NULL	colonic tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Groups 3-6 rats were given DMH at a dose of ( 20mg/kg body weight subcutaneously ) once a week for 15 weeks to induce colonic tumors .
	manualset3
83389	1	398052	5	NULL	NULL	0	NULL	Groups of Ile-de-France ewes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Groups of Ile-de-France ewes were maintained in two nutritional states ( restricted and well fed ) under a simulated annual photoperiod of 8-16 h of light per day over two breeding seasons .
	manualset3
83390	3	398052	5	NULL	NULL	NULL	NULL	simulated annual photoperiod	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Groups of Ile-de-France ewes were maintained in two nutritional states ( restricted and well fed ) under a simulated annual photoperiod of 8-16 h of light per day over two breeding seasons .
	manualset3
83391	4	398052	5	NULL	NULL	NULL	NULL	8-16 h of light per day	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Groups of Ile-de-France ewes were maintained in two nutritional states ( restricted and well fed ) under a simulated annual photoperiod of 8-16 h of light per day over two breeding seasons .
	manualset3
83392	5	398052	5	NULL	NULL	NULL	NULL	two breeding seasons	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Groups of Ile-de-France ewes were maintained in two nutritional states ( restricted and well fed ) under a simulated annual photoperiod of 8-16 h of light per day over two breeding seasons .
	manualset3
83777	2	398052	5	NULL	NULL	0	NULL	 two nutritional states ( restricted and well fed )	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Groups of Ile-de-France ewes were maintained in two nutritional states ( restricted and well fed ) under a simulated annual photoperiod of 8-16 h of light per day over two breeding seasons .
	manualset3
83393	1	398053	5	NULL	NULL	0	NULL	diatom species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Growing alone , no effect was found , but in co-culture with a single diatom species , the bacteria reduced the diatom effect on flow through the bioreactors seen earlier , however did not reduce the extent of their growth .
	manualset3
83394	2	398053	5	NULL	NULL	0	NULL	bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Growing alone , no effect was found , but in co-culture with a single diatom species , the bacteria reduced the diatom effect on flow through the bioreactors seen earlier , however did not reduce the extent of their growth .
	manualset3
83395	3	398053	5	NULL	NULL	0	NULL	diatom effect 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Growing alone , no effect was found , but in co-culture with a single diatom species , the bacteria reduced the diatom effect on flow through the bioreactors seen earlier , however did not reduce the extent of their growth .
	manualset3
83396	4	398053	5	NULL	NULL	0	NULL	bioreactors 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Growing alone , no effect was found , but in co-culture with a single diatom species , the bacteria reduced the diatom effect on flow through the bioreactors seen earlier , however did not reduce the extent of their growth .
	manualset3
83397	5	398053	5	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Growing alone , no effect was found , but in co-culture with a single diatom species , the bacteria reduced the diatom effect on flow through the bioreactors seen earlier , however did not reduce the extent of their growth .
	manualset3
83398	1	398054	5	NULL	NULL	0	NULL	Static flatfoot	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Static flatfoot in children and adolescents ) .
	manualset3
83399	2	398054	5	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Static flatfoot in children and adolescents ) .
	manualset3
83400	3	398054	5	NULL	NULL	0	NULL	adolescents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Static flatfoot in children and adolescents ) .
	manualset3
83401	1	398055	5	NULL	NULL	0	NULL	significant proportion	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Growing evidence indicates that a significant proportion of individuals with TBI demonstrate an inability to recognize affective information from the face , voice , bodily movement , and posture .
	manualset3
83402	2	398055	5	NULL	NULL	0	NULL	individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Growing evidence indicates that a significant proportion of individuals with TBI demonstrate an inability to recognize affective information from the face , voice , bodily movement , and posture .
	manualset3
83403	3	398055	5	NULL	NULL	0	NULL	TBI	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Growing evidence indicates that a significant proportion of individuals with TBI demonstrate an inability to recognize affective information from the face , voice , bodily movement , and posture .
	manualset3
83404	4	398055	5	NULL	NULL	0	NULL	recognize affective information	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Growing evidence indicates that a significant proportion of individuals with TBI demonstrate an inability to recognize affective information from the face , voice , bodily movement , and posture .
	manualset3
83405	5	398055	5	NULL	NULL	0	NULL	face	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Growing evidence indicates that a significant proportion of individuals with TBI demonstrate an inability to recognize affective information from the face , voice , bodily movement , and posture .
	manualset3
83406	6	398055	5	NULL	NULL	0	NULL	bodily movement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Growing evidence indicates that a significant proportion of individuals with TBI demonstrate an inability to recognize affective information from the face , voice , bodily movement , and posture .
	manualset3
83407	7	398055	5	NULL	NULL	0	NULL	posture	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Growing evidence indicates that a significant proportion of individuals with TBI demonstrate an inability to recognize affective information from the face , voice , bodily movement , and posture .
	manualset3
83408	1	398056	5	NULL	NULL	0	NULL	heme-mediated injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Growing evidence suggests that heme-mediated injury may contribute to the pathogenesis of CNS hemorrhage .
	manualset3
83409	2	398056	5	NULL	NULL	0	NULL	pathogenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Growing evidence suggests that heme-mediated injury may contribute to the pathogenesis of CNS hemorrhage .
	manualset3
83410	3	398056	5	NULL	NULL	0	NULL	CNS hemorrhage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Growing evidence suggests that heme-mediated injury may contribute to the pathogenesis of CNS hemorrhage .
	manualset3
83411	1	398057	5	NULL	NULL	0	NULL	Growth hormone ( GH )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth hormone ( GH ) exerts sexually dimorphic effects on liver gene transcription that are regulated by the temporal pattern of pituitary GH release ; this release is intermittent in male rats and nearly continuous in females .
	manualset3
83412	2	398057	5	NULL	NULL	0	NULL	sexually dimorphic effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth hormone ( GH ) exerts sexually dimorphic effects on liver gene transcription that are regulated by the temporal pattern of pituitary GH release ; this release is intermittent in male rats and nearly continuous in females .
	manualset3
83413	3	398057	5	NULL	NULL	0	NULL	liver gene transcription	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth hormone ( GH ) exerts sexually dimorphic effects on liver gene transcription that are regulated by the temporal pattern of pituitary GH release ; this release is intermittent in male rats and nearly continuous in females .
	manualset3
83414	4	398057	5	NULL	NULL	NULL	NULL	temporal pattern of pituitary GH release	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Growth hormone ( GH ) exerts sexually dimorphic effects on liver gene transcription that are regulated by the temporal pattern of pituitary GH release ; this release is intermittent in male rats and nearly continuous in females .
	manualset3
83415	5	398057	5	NULL	NULL	0	NULL	release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth hormone ( GH ) exerts sexually dimorphic effects on liver gene transcription that are regulated by the temporal pattern of pituitary GH release ; this release is intermittent in male rats and nearly continuous in females .
	manualset3
83416	6	398057	5	NULL	NULL	0	NULL	male rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth hormone ( GH ) exerts sexually dimorphic effects on liver gene transcription that are regulated by the temporal pattern of pituitary GH release ; this release is intermittent in male rats and nearly continuous in females .
	manualset3
83417	7	398057	5	NULL	NULL	0	NULL	females	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth hormone ( GH ) exerts sexually dimorphic effects on liver gene transcription that are regulated by the temporal pattern of pituitary GH release ; this release is intermittent in male rats and nearly continuous in females .
	manualset3
83418	1	398058	5	NULL	NULL	0	NULL	Growth hormone	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth hormone and insulin-like growth factor I regulate collagen gene expression and extracellular collagen in cultures of avian skin fibroblasts .
	manualset3
83419	2	398058	5	NULL	NULL	0	NULL	insulin-like growth factor I 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth hormone and insulin-like growth factor I regulate collagen gene expression and extracellular collagen in cultures of avian skin fibroblasts .
	manualset3
83420	3	398058	5	NULL	NULL	0	NULL	collagen gene expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth hormone and insulin-like growth factor I regulate collagen gene expression and extracellular collagen in cultures of avian skin fibroblasts .
	manualset3
83421	4	398058	5	NULL	NULL	0	NULL	extracellular collagen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth hormone and insulin-like growth factor I regulate collagen gene expression and extracellular collagen in cultures of avian skin fibroblasts .
	manualset3
83422	5	398058	5	NULL	NULL	0	NULL	cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth hormone and insulin-like growth factor I regulate collagen gene expression and extracellular collagen in cultures of avian skin fibroblasts .
	manualset3
83423	6	398058	5	NULL	NULL	0	NULL	avian skin fibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth hormone and insulin-like growth factor I regulate collagen gene expression and extracellular collagen in cultures of avian skin fibroblasts .
	manualset3
83424	1	398059	5	NULL	NULL	0	NULL	Growth hormone	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth hormone promotes early initiation of hepatocyte growth factor gene expression in the liver of hypophysectomized rats after partial hepatectomy .
	manualset3
83425	2	398059	5	NULL	NULL	0	NULL	early initiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth hormone promotes early initiation of hepatocyte growth factor gene expression in the liver of hypophysectomized rats after partial hepatectomy .
	manualset3
83426	3	398059	5	NULL	NULL	0	NULL	hepatocyte growth factor gene expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth hormone promotes early initiation of hepatocyte growth factor gene expression in the liver of hypophysectomized rats after partial hepatectomy .
	manualset3
83427	4	398059	5	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth hormone promotes early initiation of hepatocyte growth factor gene expression in the liver of hypophysectomized rats after partial hepatectomy .
	manualset3
83428	5	398059	5	NULL	NULL	0	NULL	hypophysectomized rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth hormone promotes early initiation of hepatocyte growth factor gene expression in the liver of hypophysectomized rats after partial hepatectomy .
	manualset3
83429	6	398059	5	NULL	NULL	0	NULL	partial hepatectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth hormone promotes early initiation of hepatocyte growth factor gene expression in the liver of hypophysectomized rats after partial hepatectomy .
	manualset3
83430	1	398060	5	NULL	NULL	0	NULL	Growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth in managed care enrollment potentially creates incentives for health plans to become involved in public health activities , such as health promotion and disease prevention interventions , and care for vulnerable populations .
	manualset3
83431	2	398060	5	NULL	NULL	0	NULL	managed care enrollment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth in managed care enrollment potentially creates incentives for health plans to become involved in public health activities , such as health promotion and disease prevention interventions , and care for vulnerable populations .
	manualset3
83432	3	398060	5	NULL	NULL	0	NULL	 health plans	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth in managed care enrollment potentially creates incentives for health plans to become involved in public health activities , such as health promotion and disease prevention interventions , and care for vulnerable populations .
	manualset3
83433	4	398060	5	NULL	NULL	NULL	NULL	public health activities	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Growth in managed care enrollment potentially creates incentives for health plans to become involved in public health activities , such as health promotion and disease prevention interventions , and care for vulnerable populations .
	manualset3
83434	5	398060	5	NULL	NULL	0	NULL	health promotion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth in managed care enrollment potentially creates incentives for health plans to become involved in public health activities , such as health promotion and disease prevention interventions , and care for vulnerable populations .
	manualset3
83435	6	398060	5	NULL	NULL	0	NULL	disease prevention interventions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth in managed care enrollment potentially creates incentives for health plans to become involved in public health activities , such as health promotion and disease prevention interventions , and care for vulnerable populations .
	manualset3
83436	7	398060	5	NULL	NULL	0	NULL	care	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth in managed care enrollment potentially creates incentives for health plans to become involved in public health activities , such as health promotion and disease prevention interventions , and care for vulnerable populations .
	manualset3
83437	8	398060	5	NULL	NULL	0	NULL	vulnerable populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth in managed care enrollment potentially creates incentives for health plans to become involved in public health activities , such as health promotion and disease prevention interventions , and care for vulnerable populations .
	manualset3
83438	1	398061	5	NULL	NULL	0	NULL	Growth inhibition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth inhibition was due to SE-induced programmed cell death ( apoptosis ) as shown by propidium iodide staining and the appearance of the characteristic ladder pattern of DNA fragmentation .
	manualset3
83439	2	398061	5	NULL	NULL	0	NULL	SE-induced programmed cell death ( apoptosis )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth inhibition was due to SE-induced programmed cell death ( apoptosis ) as shown by propidium iodide staining and the appearance of the characteristic ladder pattern of DNA fragmentation .
	manualset3
83440	3	398061	5	NULL	NULL	0	NULL	propidium iodide staining	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth inhibition was due to SE-induced programmed cell death ( apoptosis ) as shown by propidium iodide staining and the appearance of the characteristic ladder pattern of DNA fragmentation .
	manualset3
83441	4	398061	5	NULL	NULL	0	NULL	characteristic ladder pattern of DNA fragmentation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth inhibition was due to SE-induced programmed cell death ( apoptosis ) as shown by propidium iodide staining and the appearance of the characteristic ladder pattern of DNA fragmentation .
	manualset3
83442	1	398062	5	NULL	NULL	0	NULL	Growth patterns	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth patterns of bone marrow in complete remission from ANLL often had depressed colony numbers .
	manualset3
83443	2	398062	5	NULL	NULL	0	NULL	bone marrow	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth patterns of bone marrow in complete remission from ANLL often had depressed colony numbers .
	manualset3
83444	3	398062	5	NULL	NULL	0	NULL	complete remission	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth patterns of bone marrow in complete remission from ANLL often had depressed colony numbers .
	manualset3
83445	4	398062	5	NULL	NULL	0	NULL	ANLL	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth patterns of bone marrow in complete remission from ANLL often had depressed colony numbers .
	manualset3
83446	5	398062	5	NULL	NULL	0	NULL	depressed colony numbers	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth patterns of bone marrow in complete remission from ANLL often had depressed colony numbers .
	manualset3
83447	1	398063	5	NULL	NULL	NULL	NULL	Growth rate	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Growth rate was greater in pigs previously fed lysine-restricted diets than well-fed pigs although it did not reach a significant level during realimentation .
	manualset3
83448	2	398063	5	NULL	NULL	0	NULL	pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth rate was greater in pigs previously fed lysine-restricted diets than well-fed pigs although it did not reach a significant level during realimentation .
	manualset3
83449	3	398063	5	NULL	NULL	0	NULL	 lysine-restricted diets	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth rate was greater in pigs previously fed lysine-restricted diets than well-fed pigs although it did not reach a significant level during realimentation .
	manualset3
83450	4	398063	5	NULL	NULL	0	NULL	well-fed pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth rate was greater in pigs previously fed lysine-restricted diets than well-fed pigs although it did not reach a significant level during realimentation .
	manualset3
83451	5	398063	5	NULL	NULL	0	NULL	realimentation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth rate was greater in pigs previously fed lysine-restricted diets than well-fed pigs although it did not reach a significant level during realimentation .
	manualset3
83452	1	398064	5	NULL	NULL	0	NULL	Growth regulated peptide ( GRO-alpha ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth regulated peptide ( GRO-alpha ) is chemotactic for neutrophils .
	manualset3
83453	2	398064	5	NULL	NULL	0	NULL	neutrophils	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth regulated peptide ( GRO-alpha ) is chemotactic for neutrophils .
	manualset3
83454	1	398065	5	NULL	NULL	0	NULL	Growth stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth stimulation by NGF could be completely reversed by neutralizing anti-NGF antibody and by the tyrosine kinase inhibitor genistein .
	manualset3
83455	2	398065	5	NULL	NULL	0	NULL	NGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth stimulation by NGF could be completely reversed by neutralizing anti-NGF antibody and by the tyrosine kinase inhibitor genistein .
	manualset3
83456	3	398065	5	NULL	NULL	0	NULL	anti-NGF antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth stimulation by NGF could be completely reversed by neutralizing anti-NGF antibody and by the tyrosine kinase inhibitor genistein .
	manualset3
83457	4	398065	5	NULL	NULL	0	NULL	tyrosine kinase inhibitor genistein	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth stimulation by NGF could be completely reversed by neutralizing anti-NGF antibody and by the tyrosine kinase inhibitor genistein .
	manualset3
83458	1	398066	5	NULL	NULL	0	NULL	Growth studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth studies showed that M. pusillus had the capacity to utilize ammonium N , nitrate N , amino N , and urea .
	manualset3
83459	2	398066	5	NULL	NULL	0	NULL	M. pusillus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth studies showed that M. pusillus had the capacity to utilize ammonium N , nitrate N , amino N , and urea .
	manualset3
83460	3	398066	5	NULL	NULL	NULL	NULL	ammonium N	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Growth studies showed that M. pusillus had the capacity to utilize ammonium N , nitrate N , amino N , and urea .
	manualset3
83461	4	398066	5	NULL	NULL	NULL	NULL	nitrate N	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Growth studies showed that M. pusillus had the capacity to utilize ammonium N , nitrate N , amino N , and urea .
	manualset3
83462	5	398066	5	NULL	NULL	NULL	NULL	amino N	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Growth studies showed that M. pusillus had the capacity to utilize ammonium N , nitrate N , amino N , and urea .
	manualset3
83463	6	398066	5	NULL	NULL	0	NULL	urea	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth studies showed that M. pusillus had the capacity to utilize ammonium N , nitrate N , amino N , and urea .
	manualset3
83464	1	398067	5	NULL	NULL	0	NULL	Guanidine hydrochloride	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Guanidine hydrochloride exerts dual effects on the tryptophan synthase alpha 2 beta 2 complex as a cation activator and as a modulator of the active site conformation .
	manualset3
83465	2	398067	5	NULL	NULL	0	NULL	dual effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Guanidine hydrochloride exerts dual effects on the tryptophan synthase alpha 2 beta 2 complex as a cation activator and as a modulator of the active site conformation .
	manualset3
83466	3	398067	5	NULL	NULL	0	NULL	tryptophan synthase alpha 2 beta 2 complex	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Guanidine hydrochloride exerts dual effects on the tryptophan synthase alpha 2 beta 2 complex as a cation activator and as a modulator of the active site conformation .
	manualset3
83467	4	398067	5	NULL	NULL	0	NULL	cation activator	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Guanidine hydrochloride exerts dual effects on the tryptophan synthase alpha 2 beta 2 complex as a cation activator and as a modulator of the active site conformation .
	manualset3
83468	5	398067	5	NULL	NULL	0	NULL	 modulator of the active site conformation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Guanidine hydrochloride exerts dual effects on the tryptophan synthase alpha 2 beta 2 complex as a cation activator and as a modulator of the active site conformation .
	manualset3
83469	1	398068	5	NULL	NULL	0	NULL	Guided dilatation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Guided dilatation and transurethral resection in one session for treatment of post-prostatectomy obstructive complications .
	manualset3
83470	2	398068	5	NULL	NULL	0	NULL	transurethral resection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Guided dilatation and transurethral resection in one session for treatment of post-prostatectomy obstructive complications .
	manualset3
83471	3	398068	5	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Guided dilatation and transurethral resection in one session for treatment of post-prostatectomy obstructive complications .
	manualset3
83472	4	398068	5	NULL	NULL	0	NULL	post-prostatectomy obstructive complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Guided dilatation and transurethral resection in one session for treatment of post-prostatectomy obstructive complications .
	manualset3
83473	1	398069	5	NULL	NULL	0	NULL	guidelines	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Guidelines for establishing a maternal serum alpha-fetoprotein screening program .
	manualset3
83474	2	398069	5	NULL	NULL	0	NULL	maternal serum alpha-fetoprotein screening program	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Guidelines for establishing a maternal serum alpha-fetoprotein screening program .
	manualset3
83475	1	398070	5	NULL	NULL	0	NULL	maternal mortality	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Statistical review of maternal mortality in North-Moravian region in 1965-1974 and consequent conclusions ( author 's transl ) ) .
	manualset3
83476	2	398070	5	NULL	NULL	0	NULL	North-Moravian region	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Statistical review of maternal mortality in North-Moravian region in 1965-1974 and consequent conclusions ( author 's transl ) ) .
	manualset3
83477	3	398070	5	NULL	NULL	0	NULL	1965-1974	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	( Statistical review of maternal mortality in North-Moravian region in 1965-1974 and consequent conclusions ( author 's transl ) ) .
	manualset3
83478	1	398071	5	NULL	NULL	0	NULL	Guidelines	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Guidelines for the clinical application of the LCP .
	manualset3
83479	2	398071	5	NULL	NULL	0	NULL	clinical application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Guidelines for the clinical application of the LCP .
	manualset3
83480	3	398071	5	NULL	NULL	0	NULL	LCP	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Guidelines for the clinical application of the LCP .
	manualset3
83482	1	398072	5	NULL	NULL	0	NULL	Guidelines	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Guidelines for the documentation and verification of measles , rubella , and congenital rubella syndrome elimination in the region of the Americas .
	manualset3
83483	2	398072	5	NULL	NULL	NULL	NULL	documentation and verification	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Guidelines for the documentation and verification of measles , rubella , and congenital rubella syndrome elimination in the region of the Americas .
	manualset3
83484	3	398072	5	NULL	NULL	NULL	NULL	measles , rubella , and congenital rubella syndrome elimination	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Guidelines for the documentation and verification of measles , rubella , and congenital rubella syndrome elimination in the region of the Americas .
	manualset3
83485	4	398072	5	NULL	NULL	NULL	NULL	region	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Guidelines for the documentation and verification of measles , rubella , and congenital rubella syndrome elimination in the region of the Americas .
	manualset3
83486	5	398072	5	NULL	NULL	NULL	NULL	Americas	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Guidelines for the documentation and verification of measles , rubella , and congenital rubella syndrome elimination in the region of the Americas .
	manualset3
83487	1	398073	5	NULL	NULL	0	NULL	Guinea pig	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Guinea pig brainstem preparations possessed specific binding sites for ( 3H ) 5-HT but specific ( 3H ) spiperone binding was low and inconsistent .
	manualset3
83488	2	398073	5	NULL	NULL	0	NULL	brainstem preparations	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Guinea pig brainstem preparations possessed specific binding sites for ( 3H ) 5-HT but specific ( 3H ) spiperone binding was low and inconsistent .
	manualset3
83492	3	398073	5	NULL	NULL	0	NULL	possessed specific binding sites	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Guinea pig brainstem preparations possessed specific binding sites for ( 3H ) 5-HT but specific ( 3H ) spiperone binding was low and inconsistent .
	manualset3
83494	4	398073	5	NULL	NULL	0	NULL	( 3H ) 5-HT	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Guinea pig brainstem preparations possessed specific binding sites for ( 3H ) 5-HT but specific ( 3H ) spiperone binding was low and inconsistent .
	manualset3
83495	5	398073	5	NULL	NULL	0	NULL	specific ( 3H ) spiperone binding	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Guinea pig brainstem preparations possessed specific binding sites for ( 3H ) 5-HT but specific ( 3H ) spiperone binding was low and inconsistent .
	manualset3
83496	1	398074	5	NULL	NULL	0	NULL	Gynaecological examination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Gynaecological examination , USG and CT showed small hypoplastic uterus and rudimentary ovaries .
	manualset3
83497	2	398074	5	NULL	NULL	0	NULL	USG	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Gynaecological examination , USG and CT showed small hypoplastic uterus and rudimentary ovaries .
	manualset3
83498	3	398074	5	NULL	NULL	0	NULL	CT	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Gynaecological examination , USG and CT showed small hypoplastic uterus and rudimentary ovaries .
	manualset3
83499	4	398074	5	NULL	NULL	0	NULL	small hypoplastic uterus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gynaecological examination , USG and CT showed small hypoplastic uterus and rudimentary ovaries .
	manualset3
83500	5	398074	5	NULL	NULL	0	NULL	rudimentary ovaries	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gynaecological examination , USG and CT showed small hypoplastic uterus and rudimentary ovaries .
	manualset3
83503	1	398075	5	NULL	NULL	0	NULL	H. pylori	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	H. pylori LPS in part mediates the binding of the bacterium to laminin , and interferes with gastric cell receptor-laminin interaction , thereby potentially contributing to the loss of mucosal integrity .
	manualset3
83505	2	398075	5	NULL	NULL	0	NULL	LPS	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	H. pylori LPS in part mediates the binding of the bacterium to laminin , and interferes with gastric cell receptor-laminin interaction , thereby potentially contributing to the loss of mucosal integrity .
	manualset3
83506	3	398075	5	NULL	NULL	0	NULL	binding	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	H. pylori LPS in part mediates the binding of the bacterium to laminin , and interferes with gastric cell receptor-laminin interaction , thereby potentially contributing to the loss of mucosal integrity .
	manualset3
83508	4	398075	5	NULL	NULL	0	NULL	bacterium	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	H. pylori LPS in part mediates the binding of the bacterium to laminin , and interferes with gastric cell receptor-laminin interaction , thereby potentially contributing to the loss of mucosal integrity .
	manualset3
83509	5	398075	5	NULL	NULL	0	NULL	laminin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	H. pylori LPS in part mediates the binding of the bacterium to laminin , and interferes with gastric cell receptor-laminin interaction , thereby potentially contributing to the loss of mucosal integrity .
	manualset3
83511	6	398075	5	NULL	NULL	0	NULL	gastric cell receptor-laminin interaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	H. pylori LPS in part mediates the binding of the bacterium to laminin , and interferes with gastric cell receptor-laminin interaction , thereby potentially contributing to the loss of mucosal integrity .
	manualset3
83514	7	398075	5	NULL	NULL	0	NULL	mucosal integrity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	H. pylori LPS in part mediates the binding of the bacterium to laminin , and interferes with gastric cell receptor-laminin interaction , thereby potentially contributing to the loss of mucosal integrity .
	manualset3
83515	1	398076	5	NULL	NULL	0	NULL	H ( 2 ) O ( 2 ) production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	H ( 2 ) O ( 2 ) production and changes in glutathione , catalase , and peroxidase were followed in whole-leaf extracts from the susceptible ( AlgS ( Algerian/4 * ( F14 ) Man .
	manualset3
83516	2	398076	5	NULL	NULL	0	NULL	glutathione	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	H ( 2 ) O ( 2 ) production and changes in glutathione , catalase , and peroxidase were followed in whole-leaf extracts from the susceptible ( AlgS ( Algerian/4 * ( F14 ) Man .
	manualset3
83517	3	398076	5	NULL	NULL	0	NULL	catalase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	H ( 2 ) O ( 2 ) production and changes in glutathione , catalase , and peroxidase were followed in whole-leaf extracts from the susceptible ( AlgS ( Algerian/4 * ( F14 ) Man .
	manualset3
83518	4	398076	5	NULL	NULL	0	NULL	peroxidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	H ( 2 ) O ( 2 ) production and changes in glutathione , catalase , and peroxidase were followed in whole-leaf extracts from the susceptible ( AlgS ( Algerian/4 * ( F14 ) Man .
	manualset3
83519	5	398076	5	NULL	NULL	0	NULL	whole-leaf extracts	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	H ( 2 ) O ( 2 ) production and changes in glutathione , catalase , and peroxidase were followed in whole-leaf extracts from the susceptible ( AlgS ( Algerian/4 * ( F14 ) Man .
	manualset3
83520	6	398076	5	NULL	NULL	0	NULL	susceptible ( AlgS ( Algerian/4 * ( F14 ) Man	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	H ( 2 ) O ( 2 ) production and changes in glutathione , catalase , and peroxidase were followed in whole-leaf extracts from the susceptible ( AlgS ( Algerian/4 * ( F14 ) Man .
	manualset3
83521	1	398077	5	NULL	NULL	0	NULL	H ( 2 ) O } ( 3 )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	H ( 2 ) O } ( 3 ) , ( SbI ( 3 ) ( MTZD ) ) ( 4 ) , ( ( NMeMBZT ) SbI ( 2 ) ( mu ( 2 ) - I ) ( 2 ) ( mu ( 2 ) - S-NMeMBZT ) SbI ( 2 ) ( NMeMBZT ) ) ( 5 ) , { ( SbI ( 3 ) ( tHPMT ) ( 3 ) ) .
	manualset3
83522	2	398077	5	NULL	NULL	NULL	NULL	( SbI ( 3 ) ( MTZD ) ) ( 4 )	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	H ( 2 ) O } ( 3 ) , ( SbI ( 3 ) ( MTZD ) ) ( 4 ) , ( ( NMeMBZT ) SbI ( 2 ) ( mu ( 2 ) - I ) ( 2 ) ( mu ( 2 ) - S-NMeMBZT ) SbI ( 2 ) ( NMeMBZT ) ) ( 5 ) , { ( SbI ( 3 ) ( tHPMT ) ( 3 ) ) .
	manualset3
83524	3	398077	5	NULL	NULL	0	NULL	( ( NMeMBZT ) SbI ( 2 ) ( mu ( 2 ) - I ) ( 2 ) ( mu ( 2 ) - S-NMeMBZT ) SbI ( 2 ) ( NMeMBZT ) ) ( 5 ) 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	H ( 2 ) O } ( 3 ) , ( SbI ( 3 ) ( MTZD ) ) ( 4 ) , ( ( NMeMBZT ) SbI ( 2 ) ( mu ( 2 ) - I ) ( 2 ) ( mu ( 2 ) - S-NMeMBZT ) SbI ( 2 ) ( NMeMBZT ) ) ( 5 ) , { ( SbI ( 3 ) ( tHPMT ) ( 3 ) ) .
	manualset3
83526	4	398077	5	NULL	NULL	0	NULL	{ ( SbI ( 3 ) ( tHPMT ) ( 3 ) )	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	H ( 2 ) O } ( 3 ) , ( SbI ( 3 ) ( MTZD ) ) ( 4 ) , ( ( NMeMBZT ) SbI ( 2 ) ( mu ( 2 ) - I ) ( 2 ) ( mu ( 2 ) - S-NMeMBZT ) SbI ( 2 ) ( NMeMBZT ) ) ( 5 ) , { ( SbI ( 3 ) ( tHPMT ) ( 3 ) ) .
	manualset3
83528	1	398078	5	NULL	NULL	0	NULL	Alpha-fetoprotein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Alpha-fetoprotein ( author 's transl ) ) .
	manualset3
83529	1	398079	5	NULL	NULL	NULL	NULL	H complex concentration	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	H complex concentration was found up to 25 microM whether the reaction was followed by probe displacement or the quenching of AT .
	manualset3
83530	2	398079	5	NULL	NULL	0	NULL	25 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	H complex concentration was found up to 25 microM whether the reaction was followed by probe displacement or the quenching of AT .
	manualset3
83531	3	398079	5	NULL	NULL	0	NULL	reaction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	H complex concentration was found up to 25 microM whether the reaction was followed by probe displacement or the quenching of AT .
	manualset3
83532	4	398079	5	NULL	NULL	NULL	NULL	probe displacement	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	H complex concentration was found up to 25 microM whether the reaction was followed by probe displacement or the quenching of AT .
	manualset3
83533	5	398079	5	NULL	NULL	0	NULL	quenching of AT	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	H complex concentration was found up to 25 microM whether the reaction was followed by probe displacement or the quenching of AT .
	manualset3
83534	1	398080	5	NULL	NULL	0	NULL	H pylori infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	H pylori infection was detected in 85 % of patients versus 76.7 % for control subjects .
	manualset3
83535	2	398080	5	NULL	NULL	0	NULL	85 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	H pylori infection was detected in 85 % of patients versus 76.7 % for control subjects .
	manualset3
83537	3	398080	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	H pylori infection was detected in 85 % of patients versus 76.7 % for control subjects .
	manualset3
83538	4	398080	5	NULL	NULL	0	NULL	76.7 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	H pylori infection was detected in 85 % of patients versus 76.7 % for control subjects .
	manualset3
83539	5	398080	5	NULL	NULL	0	NULL	control subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	H pylori infection was detected in 85 % of patients versus 76.7 % for control subjects .
	manualset3
83540	1	398081	5	NULL	NULL	0	NULL	H2-M	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	H2-M , a facilitator of MHC class II peptide loading , and its negative modulator H2-O are differentially expressed in response to proinflammatory cytokines .
	manualset3
83541	2	398081	5	NULL	NULL	0	NULL	facilitator 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	H2-M , a facilitator of MHC class II peptide loading , and its negative modulator H2-O are differentially expressed in response to proinflammatory cytokines .
	manualset3
83542	3	398081	5	NULL	NULL	0	NULL	MHC class II peptide loading	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	H2-M , a facilitator of MHC class II peptide loading , and its negative modulator H2-O are differentially expressed in response to proinflammatory cytokines .
	manualset3
83543	4	398081	5	NULL	NULL	0	NULL	negative modulator H2-O	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	H2-M , a facilitator of MHC class II peptide loading , and its negative modulator H2-O are differentially expressed in response to proinflammatory cytokines .
	manualset3
83544	5	398081	5	NULL	NULL	0	NULL	response 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	H2-M , a facilitator of MHC class II peptide loading , and its negative modulator H2-O are differentially expressed in response to proinflammatory cytokines .
	manualset3
83545	6	398081	5	NULL	NULL	0	NULL	proinflammatory cytokines	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	H2-M , a facilitator of MHC class II peptide loading , and its negative modulator H2-O are differentially expressed in response to proinflammatory cytokines .
	manualset3
83548	1	398082	5	NULL	NULL	NULL	NULL	H2mfpp	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	H2mfpp and its complexes Sn ( Hmfpp ) ( C2H5 ) 2Cl and Sn3 ( Hmfpp ) ( mfpp ) ( C6H5 ) 3Cl6 are shown by the Salmonella-microsome assay to be mutagenic substances in the presence of a metabolic activation system .
	manualset3
83549	2	398082	5	NULL	NULL	NULL	NULL	Sn ( Hmfpp ) ( C2H5 ) 2Cl	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	H2mfpp and its complexes Sn ( Hmfpp ) ( C2H5 ) 2Cl and Sn3 ( Hmfpp ) ( mfpp ) ( C6H5 ) 3Cl6 are shown by the Salmonella-microsome assay to be mutagenic substances in the presence of a metabolic activation system .
	manualset3
83550	3	398082	5	NULL	NULL	0	NULL	Sn3 ( Hmfpp ) ( mfpp ) ( C6H5 ) 3Cl6	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	H2mfpp and its complexes Sn ( Hmfpp ) ( C2H5 ) 2Cl and Sn3 ( Hmfpp ) ( mfpp ) ( C6H5 ) 3Cl6 are shown by the Salmonella-microsome assay to be mutagenic substances in the presence of a metabolic activation system .
	manualset3
83552	4	398082	5	NULL	NULL	0	NULL	Salmonella-microsome assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	H2mfpp and its complexes Sn ( Hmfpp ) ( C2H5 ) 2Cl and Sn3 ( Hmfpp ) ( mfpp ) ( C6H5 ) 3Cl6 are shown by the Salmonella-microsome assay to be mutagenic substances in the presence of a metabolic activation system .
	manualset3
83553	5	398082	5	NULL	NULL	0	NULL	mutagenic substances	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	H2mfpp and its complexes Sn ( Hmfpp ) ( C2H5 ) 2Cl and Sn3 ( Hmfpp ) ( mfpp ) ( C6H5 ) 3Cl6 are shown by the Salmonella-microsome assay to be mutagenic substances in the presence of a metabolic activation system .
	manualset3
83554	6	398082	5	NULL	NULL	0	NULL	metabolic activation system	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	H2mfpp and its complexes Sn ( Hmfpp ) ( C2H5 ) 2Cl and Sn3 ( Hmfpp ) ( mfpp ) ( C6H5 ) 3Cl6 are shown by the Salmonella-microsome assay to be mutagenic substances in the presence of a metabolic activation system .
	manualset3
83557	1	398083	5	NULL	NULL	0	NULL	H3 .3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	H3 .3 is also incorporated during decondensation of the Drosophila sperm pronucleus , indicating a direct role in chromatin remodeling upon fertilization .
	manualset3
83559	2	398083	5	NULL	NULL	0	NULL	decondensation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	H3 .3 is also incorporated during decondensation of the Drosophila sperm pronucleus , indicating a direct role in chromatin remodeling upon fertilization .
	manualset3
83560	3	398083	5	NULL	NULL	0	NULL	Drosophila sperm pronucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	H3 .3 is also incorporated during decondensation of the Drosophila sperm pronucleus , indicating a direct role in chromatin remodeling upon fertilization .
	manualset3
83562	4	398083	5	NULL	NULL	0	NULL	direct role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	H3 .3 is also incorporated during decondensation of the Drosophila sperm pronucleus , indicating a direct role in chromatin remodeling upon fertilization .
	manualset3
83563	5	398083	5	NULL	NULL	0	NULL	chromatin remodeling	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	H3 .3 is also incorporated during decondensation of the Drosophila sperm pronucleus , indicating a direct role in chromatin remodeling upon fertilization .
	manualset3
83565	6	398083	5	NULL	NULL	0	NULL	fertilization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	H3 .3 is also incorporated during decondensation of the Drosophila sperm pronucleus , indicating a direct role in chromatin remodeling upon fertilization .
	manualset3
83566	1	398084	5	NULL	NULL	0	NULL	HABC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	HABC responded better than HPC and HGF to CAP treated root slices , and HPC response was higher than that of HGF .
	manualset3
83567	2	398084	5	NULL	NULL	0	NULL	HPC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	HABC responded better than HPC and HGF to CAP treated root slices , and HPC response was higher than that of HGF .
	manualset3
83568	3	398084	5	NULL	NULL	0	NULL	HGF	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	HABC responded better than HPC and HGF to CAP treated root slices , and HPC response was higher than that of HGF .
	manualset3
83570	4	398084	5	NULL	NULL	0	NULL	CAP treated root slices	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	HABC responded better than HPC and HGF to CAP treated root slices , and HPC response was higher than that of HGF .
	manualset3
83571	5	398084	5	NULL	NULL	0	NULL	HPC response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HABC responded better than HPC and HGF to CAP treated root slices , and HPC response was higher than that of HGF .
	manualset3
83573	6	398084	5	NULL	NULL	0	NULL	HGF	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	HABC responded better than HPC and HGF to CAP treated root slices , and HPC response was higher than that of HGF .
	manualset3
83575	1	398085	5	NULL	NULL	0	NULL	HAVAb 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	HAVAb was in 75 % of the cases , its meaning was of post-contact with HAV .
	manualset3
83576	2	398085	5	NULL	NULL	0	NULL	75 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	HAVAb was in 75 % of the cases , its meaning was of post-contact with HAV .
	manualset3
83587	3	398085	5	NULL	NULL	0	NULL	post-contact	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HAVAb was in 75 % of the cases , its meaning was of post-contact with HAV .
	manualset3
83588	4	398085	5	NULL	NULL	0	NULL	HAV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	HAVAb was in 75 % of the cases , its meaning was of post-contact with HAV .
	manualset3
83591	1	398086	5	NULL	NULL	0	NULL	HBO	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	HBO was most effective when whole-body and regional hypoxia was applied simultaneously .
	manualset3
83594	2	398086	5	NULL	NULL	0	NULL	whole-body	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	HBO was most effective when whole-body and regional hypoxia was applied simultaneously .
	manualset3
83595	3	398086	5	NULL	NULL	0	NULL	regional hypoxia	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HBO was most effective when whole-body and regional hypoxia was applied simultaneously .
	manualset3
83596	1	398087	5	NULL	NULL	NULL	NULL	psychotherapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Status of the psychotherapy in general practice ? ) .
	manualset3
83597	2	398087	5	NULL	NULL	0	NULL	general practice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Status of the psychotherapy in general practice ? ) .
	manualset3
83598	1	398088	5	NULL	NULL	0	NULL	HBV-related hepatocellular carcinoma susceptibility gene KIF1B	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	HBV-related hepatocellular carcinoma susceptibility gene KIF1B is not associated with development of chronic hepatitis B .
	manualset3
83599	2	398088	5	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HBV-related hepatocellular carcinoma susceptibility gene KIF1B is not associated with development of chronic hepatitis B .
	manualset3
83601	3	398088	5	NULL	NULL	0	NULL	chronic hepatitis B	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	HBV-related hepatocellular carcinoma susceptibility gene KIF1B is not associated with development of chronic hepatitis B .
	manualset3
83602	1	398089	5	NULL	NULL	0	NULL	HCC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	HCC recurred after an occlusion of the reservoir in 18 patients .
	manualset3
83603	2	398089	5	NULL	NULL	NULL	NULL	occlusion of the reservoir	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	HCC recurred after an occlusion of the reservoir in 18 patients .
	manualset3
83604	3	398089	5	NULL	NULL	NULL	NULL	18 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	HCC recurred after an occlusion of the reservoir in 18 patients .
	manualset3
83605	1	398090	5	NULL	NULL	0	NULL	HCF-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	HCF-1 is a highly conserved and abundant chromatin-associated host cell factor required for transcriptional activation of herpes simplex virus immediate-early genes by the virion protein VP16 .
	manualset3
83606	2	398090	5	NULL	NULL	0	NULL	highly conserved and abundant chromatin-associated host cell factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	HCF-1 is a highly conserved and abundant chromatin-associated host cell factor required for transcriptional activation of herpes simplex virus immediate-early genes by the virion protein VP16 .
	manualset3
83607	3	398090	5	NULL	NULL	0	NULL	transcriptional activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HCF-1 is a highly conserved and abundant chromatin-associated host cell factor required for transcriptional activation of herpes simplex virus immediate-early genes by the virion protein VP16 .
	manualset3
83608	4	398090	5	NULL	NULL	0	NULL	herpes simplex virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	HCF-1 is a highly conserved and abundant chromatin-associated host cell factor required for transcriptional activation of herpes simplex virus immediate-early genes by the virion protein VP16 .
	manualset3
83609	5	398090	5	NULL	NULL	0	NULL	immediate-early genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	HCF-1 is a highly conserved and abundant chromatin-associated host cell factor required for transcriptional activation of herpes simplex virus immediate-early genes by the virion protein VP16 .
	manualset3
83610	6	398090	5	NULL	NULL	0	NULL	virion protein VP16	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	HCF-1 is a highly conserved and abundant chromatin-associated host cell factor required for transcriptional activation of herpes simplex virus immediate-early genes by the virion protein VP16 .
	manualset3
83611	1	398091	5	NULL	NULL	0	NULL	HCMV infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	HCMV infection resulted in increased Sp1 mRNA expression , protein levels , and DNA binding activity .
	manualset3
83612	2	398091	5	NULL	NULL	0	NULL	Sp1 mRNA expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HCMV infection resulted in increased Sp1 mRNA expression , protein levels , and DNA binding activity .
	manualset3
83613	3	398091	5	NULL	NULL	0	NULL	protein levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	HCMV infection resulted in increased Sp1 mRNA expression , protein levels , and DNA binding activity .
	manualset3
83614	4	398091	5	NULL	NULL	0	NULL	DNA binding activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HCMV infection resulted in increased Sp1 mRNA expression , protein levels , and DNA binding activity .
	manualset3
83615	1	398092	5	NULL	NULL	0	NULL	HDAC8	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	HDAC8 enhanced endocytosis , acidification , and penetration of the incoming virus .
	manualset3
83616	2	398092	5	NULL	NULL	0	NULL	endocytosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HDAC8 enhanced endocytosis , acidification , and penetration of the incoming virus .
	manualset3
83617	3	398092	5	NULL	NULL	0	NULL	acidification 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HDAC8 enhanced endocytosis , acidification , and penetration of the incoming virus .
	manualset3
83618	4	398092	5	NULL	NULL	0	NULL	penetration 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HDAC8 enhanced endocytosis , acidification , and penetration of the incoming virus .
	manualset3
83619	5	398092	5	NULL	NULL	0	NULL	incoming virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	HDAC8 enhanced endocytosis , acidification , and penetration of the incoming virus .
	manualset3
83620	1	398093	5	NULL	NULL	0	NULL	HDL-C : LDL-C ratios	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	HDL-C : LDL-C ratios increased significantly in the estrogen and raloxifene groups ( range 9-29 % ) .
	manualset3
83621	2	398093	5	NULL	NULL	NULL	NULL	estrogen and raloxifene groups	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	HDL-C : LDL-C ratios increased significantly in the estrogen and raloxifene groups ( range 9-29 % ) .
	manualset3
83622	3	398093	5	NULL	NULL	0	NULL	range 9-29 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	HDL-C : LDL-C ratios increased significantly in the estrogen and raloxifene groups ( range 9-29 % ) .
	manualset3
83623	1	398094	5	NULL	NULL	0	NULL	Stem cell regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Stem cell regulation in plants ) .
	manualset3
83624	2	398094	5	NULL	NULL	0	NULL	plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Stem cell regulation in plants ) .
	manualset3
83625	1	398095	5	NULL	NULL	0	NULL	HER-2 / neu-overexpressing breast cancer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	HER-2 / neu-overexpressing breast cancer cells are more resistant to the chemotherapeutic agent paclitaxel ( Taxol ) than low-HER-2 / neu-expressing breast cancer cells , and the adenoviral type 5 EIA can down-regulate HER-2 / neu overexpression .
	manualset3
83626	2	398095	5	NULL	NULL	0	NULL	resistant	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HER-2 / neu-overexpressing breast cancer cells are more resistant to the chemotherapeutic agent paclitaxel ( Taxol ) than low-HER-2 / neu-expressing breast cancer cells , and the adenoviral type 5 EIA can down-regulate HER-2 / neu overexpression .
	manualset3
83627	3	398095	5	NULL	NULL	0	NULL	chemotherapeutic agent paclitaxel ( Taxol )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	HER-2 / neu-overexpressing breast cancer cells are more resistant to the chemotherapeutic agent paclitaxel ( Taxol ) than low-HER-2 / neu-expressing breast cancer cells , and the adenoviral type 5 EIA can down-regulate HER-2 / neu overexpression .
	manualset3
83628	4	398095	5	NULL	NULL	0	NULL	low-HER-2 / neu-expressing breast cancer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	HER-2 / neu-overexpressing breast cancer cells are more resistant to the chemotherapeutic agent paclitaxel ( Taxol ) than low-HER-2 / neu-expressing breast cancer cells , and the adenoviral type 5 EIA can down-regulate HER-2 / neu overexpression .
	manualset3
83629	5	398095	5	NULL	NULL	0	NULL	adenoviral type 5 EIA	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	HER-2 / neu-overexpressing breast cancer cells are more resistant to the chemotherapeutic agent paclitaxel ( Taxol ) than low-HER-2 / neu-expressing breast cancer cells , and the adenoviral type 5 EIA can down-regulate HER-2 / neu overexpression .
	manualset3
83630	6	398095	5	NULL	NULL	0	NULL	HER-2 / neu overexpression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HER-2 / neu-overexpressing breast cancer cells are more resistant to the chemotherapeutic agent paclitaxel ( Taxol ) than low-HER-2 / neu-expressing breast cancer cells , and the adenoviral type 5 EIA can down-regulate HER-2 / neu overexpression .
	manualset3
83631	1	398096	5	NULL	NULL	0	NULL	HERV ( Human Endogenous Retrovirus )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	HERV ( Human Endogenous Retrovirus ) - encoded envelope proteins are implicated in the development of the placenta .
	manualset3
83632	2	398096	5	NULL	NULL	0	NULL	envelope proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	HERV ( Human Endogenous Retrovirus ) - encoded envelope proteins are implicated in the development of the placenta .
	manualset3
83633	3	398096	5	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HERV ( Human Endogenous Retrovirus ) - encoded envelope proteins are implicated in the development of the placenta .
	manualset3
83634	4	398096	5	NULL	NULL	0	NULL	placenta	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	HERV ( Human Endogenous Retrovirus ) - encoded envelope proteins are implicated in the development of the placenta .
	manualset3
83635	1	398097	5	NULL	NULL	0	NULL	HEW-NIH dtente	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	HEW-NIH dtente , plus other matters .
	manualset3
83636	1	398098	5	NULL	NULL	0	NULL	HEX1-N2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	HEX1-N2 is approximately 3-fold less active in Mn ( 2 + ) - containing buffers and exhibits & lt ; 5 % activity in the presence of Co ( 2 + ) , Zn ( 2 + ) , or Ca ( 2 + ) .
	manualset3
83637	2	398098	5	NULL	NULL	0	NULL	3-fold less active	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	HEX1-N2 is approximately 3-fold less active in Mn ( 2 + ) - containing buffers and exhibits & lt ; 5 % activity in the presence of Co ( 2 + ) , Zn ( 2 + ) , or Ca ( 2 + ) .
	manualset3
83638	3	398098	5	NULL	NULL	0	NULL	Mn ( 2 + ) - containing buffers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	HEX1-N2 is approximately 3-fold less active in Mn ( 2 + ) - containing buffers and exhibits & lt ; 5 % activity in the presence of Co ( 2 + ) , Zn ( 2 + ) , or Ca ( 2 + ) .
	manualset3
83639	4	398098	5	NULL	NULL	0	NULL	5 % activity	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	HEX1-N2 is approximately 3-fold less active in Mn ( 2 + ) - containing buffers and exhibits & lt ; 5 % activity in the presence of Co ( 2 + ) , Zn ( 2 + ) , or Ca ( 2 + ) .
	manualset3
83640	5	398098	5	NULL	NULL	0	NULL	Co ( 2 + )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	HEX1-N2 is approximately 3-fold less active in Mn ( 2 + ) - containing buffers and exhibits & lt ; 5 % activity in the presence of Co ( 2 + ) , Zn ( 2 + ) , or Ca ( 2 + ) .
	manualset3
83641	6	398098	5	NULL	NULL	0	NULL	Zn ( 2 + )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	HEX1-N2 is approximately 3-fold less active in Mn ( 2 + ) - containing buffers and exhibits & lt ; 5 % activity in the presence of Co ( 2 + ) , Zn ( 2 + ) , or Ca ( 2 + ) .
	manualset3
83642	7	398098	5	NULL	NULL	0	NULL	Ca ( 2 + )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	HEX1-N2 is approximately 3-fold less active in Mn ( 2 + ) - containing buffers and exhibits & lt ; 5 % activity in the presence of Co ( 2 + ) , Zn ( 2 + ) , or Ca ( 2 + ) .
	manualset3
83643	1	398099	5	NULL	NULL	0	NULL	HEp-2 cell monolayers	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	HEp-2 cell monolayers were cocultured with intracellular Staphylococcus aureus , and changes in gene expression were profiled using DNA microarrays .
	manualset3
83644	2	398099	5	NULL	NULL	0	NULL	intracellular Staphylococcus aureus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	HEp-2 cell monolayers were cocultured with intracellular Staphylococcus aureus , and changes in gene expression were profiled using DNA microarrays .
	manualset3
83645	3	398099	5	NULL	NULL	0	NULL	changes in gene expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HEp-2 cell monolayers were cocultured with intracellular Staphylococcus aureus , and changes in gene expression were profiled using DNA microarrays .
	manualset3
83646	4	398099	5	NULL	NULL	0	NULL	DNA microarrays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	HEp-2 cell monolayers were cocultured with intracellular Staphylococcus aureus , and changes in gene expression were profiled using DNA microarrays .
	manualset3
83647	1	398100	5	NULL	NULL	0	NULL	HG stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HG stimulation of VEGF synthesis is prevented by captopril , an inhibitor of angiotensin-converting enzyme , and , by losartan , a specific antagonist of angiotensin type 1 receptor ( AT1 ) , suggesting that VEGF synthesis is mediated by Ang II .
	manualset3
83648	2	398100	5	NULL	NULL	0	NULL	VEGF synthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HG stimulation of VEGF synthesis is prevented by captopril , an inhibitor of angiotensin-converting enzyme , and , by losartan , a specific antagonist of angiotensin type 1 receptor ( AT1 ) , suggesting that VEGF synthesis is mediated by Ang II .
	manualset3
83649	3	398100	5	NULL	NULL	0	NULL	captopril 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	HG stimulation of VEGF synthesis is prevented by captopril , an inhibitor of angiotensin-converting enzyme , and , by losartan , a specific antagonist of angiotensin type 1 receptor ( AT1 ) , suggesting that VEGF synthesis is mediated by Ang II .
	manualset3
83650	4	398100	5	NULL	NULL	0	NULL	inhibitor of angiotensin-converting enzyme	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	HG stimulation of VEGF synthesis is prevented by captopril , an inhibitor of angiotensin-converting enzyme , and , by losartan , a specific antagonist of angiotensin type 1 receptor ( AT1 ) , suggesting that VEGF synthesis is mediated by Ang II .
	manualset3
83651	5	398100	5	NULL	NULL	0	NULL	losartan	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	HG stimulation of VEGF synthesis is prevented by captopril , an inhibitor of angiotensin-converting enzyme , and , by losartan , a specific antagonist of angiotensin type 1 receptor ( AT1 ) , suggesting that VEGF synthesis is mediated by Ang II .
	manualset3
83652	6	398100	5	NULL	NULL	0	NULL	specific antagonist of angiotensin type 1 receptor ( AT1 ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	HG stimulation of VEGF synthesis is prevented by captopril , an inhibitor of angiotensin-converting enzyme , and , by losartan , a specific antagonist of angiotensin type 1 receptor ( AT1 ) , suggesting that VEGF synthesis is mediated by Ang II .
	manualset3
83653	7	398100	5	NULL	NULL	0	NULL	VEGF synthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HG stimulation of VEGF synthesis is prevented by captopril , an inhibitor of angiotensin-converting enzyme , and , by losartan , a specific antagonist of angiotensin type 1 receptor ( AT1 ) , suggesting that VEGF synthesis is mediated by Ang II .
	manualset3
83654	8	398100	5	NULL	NULL	0	NULL	Ang II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	HG stimulation of VEGF synthesis is prevented by captopril , an inhibitor of angiotensin-converting enzyme , and , by losartan , a specific antagonist of angiotensin type 1 receptor ( AT1 ) , suggesting that VEGF synthesis is mediated by Ang II .
	manualset3
83655	1	398101	5	NULL	NULL	0	NULL	HGF mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	HGF mRNA was elevated following obstruction and showed increased expression 1 day after decompression , peaking at 2 days of repair .
	manualset3
83656	2	398101	5	NULL	NULL	0	NULL	obstruction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	HGF mRNA was elevated following obstruction and showed increased expression 1 day after decompression , peaking at 2 days of repair .
	manualset3
83657	3	398101	5	NULL	NULL	0	NULL	increased expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HGF mRNA was elevated following obstruction and showed increased expression 1 day after decompression , peaking at 2 days of repair .
	manualset3
83658	4	398101	5	NULL	NULL	0	NULL	1 day	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	HGF mRNA was elevated following obstruction and showed increased expression 1 day after decompression , peaking at 2 days of repair .
	manualset3
83659	5	398101	5	NULL	NULL	NULL	NULL	decompression 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	HGF mRNA was elevated following obstruction and showed increased expression 1 day after decompression , peaking at 2 days of repair .
	manualset3
83660	6	398101	5	NULL	NULL	0	NULL	2 days	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	HGF mRNA was elevated following obstruction and showed increased expression 1 day after decompression , peaking at 2 days of repair .
	manualset3
83661	7	398101	5	NULL	NULL	0	NULL	repair	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HGF mRNA was elevated following obstruction and showed increased expression 1 day after decompression , peaking at 2 days of repair .
	manualset3
83662	1	398102	5	NULL	NULL	0	NULL	HIF-1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	HIF-1 and mechanisms of hypoxia sensing .
	manualset3
83663	2	398102	5	NULL	NULL	NULL	NULL	mechanisms	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	HIF-1 and mechanisms of hypoxia sensing .
	manualset3
83664	3	398102	5	NULL	NULL	0	NULL	hypoxia sensing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HIF-1 and mechanisms of hypoxia sensing .
	manualset3
83665	1	398103	5	NULL	NULL	0	NULL	Stiff man syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Stiff man syndrome ( Moersch and Woltman syndrome ) .
	manualset3
83666	2	398103	5	NULL	NULL	0	NULL	Moersch and Woltman syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Stiff man syndrome ( Moersch and Woltman syndrome ) .
	manualset3
83667	1	398104	5	NULL	NULL	0	NULL	HIV-1	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	HIV-1 acquires resistance to two classes of antiviral drugs through homologous recombination .
	manualset3
83668	2	398104	5	NULL	NULL	0	NULL	resistance 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HIV-1 acquires resistance to two classes of antiviral drugs through homologous recombination .
	manualset3
83669	3	398104	5	NULL	NULL	0	NULL	antiviral drugs	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	HIV-1 acquires resistance to two classes of antiviral drugs through homologous recombination .
	manualset3
83670	4	398104	5	NULL	NULL	0	NULL	homologous recombination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HIV-1 acquires resistance to two classes of antiviral drugs through homologous recombination .
	manualset3
83671	1	398105	5	NULL	NULL	0	NULL	HIV-1 transcription	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HIV-1 transcription is activated by HIV-1 Tat protein , which recruits cyclin-dependent kinase 9 ( CDK9 ) / cyclin T1 and other host transcriptional coactivators to the HIV-1 promoter .
	manualset3
83672	2	398105	5	NULL	NULL	0	NULL	HIV-1 Tat protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	HIV-1 transcription is activated by HIV-1 Tat protein , which recruits cyclin-dependent kinase 9 ( CDK9 ) / cyclin T1 and other host transcriptional coactivators to the HIV-1 promoter .
	manualset3
83673	3	398105	5	NULL	NULL	0	NULL	cyclin-dependent kinase 9 ( CDK9 ) / cyclin T1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	HIV-1 transcription is activated by HIV-1 Tat protein , which recruits cyclin-dependent kinase 9 ( CDK9 ) / cyclin T1 and other host transcriptional coactivators to the HIV-1 promoter .
	manualset3
83674	4	398105	5	NULL	NULL	0	NULL	host transcriptional coactivators	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	HIV-1 transcription is activated by HIV-1 Tat protein , which recruits cyclin-dependent kinase 9 ( CDK9 ) / cyclin T1 and other host transcriptional coactivators to the HIV-1 promoter .
	manualset3
83675	5	398105	5	NULL	NULL	0	NULL	HIV-1 promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	HIV-1 transcription is activated by HIV-1 Tat protein , which recruits cyclin-dependent kinase 9 ( CDK9 ) / cyclin T1 and other host transcriptional coactivators to the HIV-1 promoter .
	manualset3
83676	1	398106	5	NULL	NULL	0	NULL	HIV infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	HIV infection : treatment outcomes in older and younger adults .
	manualset3
83677	2	398106	5	NULL	NULL	0	NULL	treatment outcomes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	HIV infection : treatment outcomes in older and younger adults .
	manualset3
83678	3	398106	5	NULL	NULL	0	NULL	older and younger adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	HIV infection : treatment outcomes in older and younger adults .
	manualset3
83679	1	398107	5	NULL	NULL	0	NULL	HIV transmission	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HIV transmission has been facilitated by ( a ) concomitant sexually transmitted diseases ( STDs ) , ( b ) the presence of social conditions that create core groups who have frequent and numerous partners , ( c ) sexual practices associated with bleeding ( i.e. , trauma , sex during menses ) as well as noncircumcision , ( d ) cervical ectopy , and ( e ) anal sex .
	manualset3
83680	2	398107	5	NULL	NULL	0	NULL	concomitant sexually transmitted diseases ( STDs )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	HIV transmission has been facilitated by ( a ) concomitant sexually transmitted diseases ( STDs ) , ( b ) the presence of social conditions that create core groups who have frequent and numerous partners , ( c ) sexual practices associated with bleeding ( i.e. , trauma , sex during menses ) as well as noncircumcision , ( d ) cervical ectopy , and ( e ) anal sex .
	manualset3
83681	3	398107	5	NULL	NULL	NULL	NULL	social conditions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	HIV transmission has been facilitated by ( a ) concomitant sexually transmitted diseases ( STDs ) , ( b ) the presence of social conditions that create core groups who have frequent and numerous partners , ( c ) sexual practices associated with bleeding ( i.e. , trauma , sex during menses ) as well as noncircumcision , ( d ) cervical ectopy , and ( e ) anal sex .
	manualset3
83682	4	398107	5	NULL	NULL	0	NULL	core groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	HIV transmission has been facilitated by ( a ) concomitant sexually transmitted diseases ( STDs ) , ( b ) the presence of social conditions that create core groups who have frequent and numerous partners , ( c ) sexual practices associated with bleeding ( i.e. , trauma , sex during menses ) as well as noncircumcision , ( d ) cervical ectopy , and ( e ) anal sex .
	manualset3
83683	5	398107	5	NULL	NULL	0	NULL	frequent and numerous partners	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	HIV transmission has been facilitated by ( a ) concomitant sexually transmitted diseases ( STDs ) , ( b ) the presence of social conditions that create core groups who have frequent and numerous partners , ( c ) sexual practices associated with bleeding ( i.e. , trauma , sex during menses ) as well as noncircumcision , ( d ) cervical ectopy , and ( e ) anal sex .
	manualset3
83684	6	398107	5	NULL	NULL	NULL	NULL	sexual practices associated with bleeding	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	HIV transmission has been facilitated by ( a ) concomitant sexually transmitted diseases ( STDs ) , ( b ) the presence of social conditions that create core groups who have frequent and numerous partners , ( c ) sexual practices associated with bleeding ( i.e. , trauma , sex during menses ) as well as noncircumcision , ( d ) cervical ectopy , and ( e ) anal sex .
	manualset3
83686	7	398107	5	NULL	NULL	NULL	NULL	trauma	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	HIV transmission has been facilitated by ( a ) concomitant sexually transmitted diseases ( STDs ) , ( b ) the presence of social conditions that create core groups who have frequent and numerous partners , ( c ) sexual practices associated with bleeding ( i.e. , trauma , sex during menses ) as well as noncircumcision , ( d ) cervical ectopy , and ( e ) anal sex .
	manualset3
83687	8	398107	5	NULL	NULL	NULL	NULL	sex during menses	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	HIV transmission has been facilitated by ( a ) concomitant sexually transmitted diseases ( STDs ) , ( b ) the presence of social conditions that create core groups who have frequent and numerous partners , ( c ) sexual practices associated with bleeding ( i.e. , trauma , sex during menses ) as well as noncircumcision , ( d ) cervical ectopy , and ( e ) anal sex .
	manualset3
83689	9	398107	5	NULL	NULL	NULL	NULL	noncircumcision	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	HIV transmission has been facilitated by ( a ) concomitant sexually transmitted diseases ( STDs ) , ( b ) the presence of social conditions that create core groups who have frequent and numerous partners , ( c ) sexual practices associated with bleeding ( i.e. , trauma , sex during menses ) as well as noncircumcision , ( d ) cervical ectopy , and ( e ) anal sex .
	manualset3
83690	10	398107	5	NULL	NULL	NULL	NULL	cervical ectopy	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	HIV transmission has been facilitated by ( a ) concomitant sexually transmitted diseases ( STDs ) , ( b ) the presence of social conditions that create core groups who have frequent and numerous partners , ( c ) sexual practices associated with bleeding ( i.e. , trauma , sex during menses ) as well as noncircumcision , ( d ) cervical ectopy , and ( e ) anal sex .
	manualset3
83691	11	398107	5	NULL	NULL	NULL	NULL	anal sex	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	HIV transmission has been facilitated by ( a ) concomitant sexually transmitted diseases ( STDs ) , ( b ) the presence of social conditions that create core groups who have frequent and numerous partners , ( c ) sexual practices associated with bleeding ( i.e. , trauma , sex during menses ) as well as noncircumcision , ( d ) cervical ectopy , and ( e ) anal sex .
	manualset3
83692	1	398108	5	NULL	NULL	0	NULL	HLA allotyping	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	HLA allotyping strongly suggested C2 depression associated with a C4BQ0 allele .
	manualset3
83693	2	398108	5	NULL	NULL	0	NULL	C2 depression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	HLA allotyping strongly suggested C2 depression associated with a C4BQ0 allele .
	manualset3
83694	3	398108	5	NULL	NULL	0	NULL	C4BQ0 allele	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	HLA allotyping strongly suggested C2 depression associated with a C4BQ0 allele .
	manualset3
83695	1	398109	5	NULL	NULL	0	NULL	HLA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	HLA is the most informative system in all three populations , followed by PGM1 , with the rhesus blood group the next most useful in the whites and ` coloured 's , whereas ABO is the next most useful in the blacks .
	manualset3
83697	2	398109	5	NULL	NULL	NULL	NULL	three populations	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	HLA is the most informative system in all three populations , followed by PGM1 , with the rhesus blood group the next most useful in the whites and ` coloured 's , whereas ABO is the next most useful in the blacks .
	manualset3
83698	3	398109	5	NULL	NULL	NULL	NULL	PGM1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	HLA is the most informative system in all three populations , followed by PGM1 , with the rhesus blood group the next most useful in the whites and ` coloured 's , whereas ABO is the next most useful in the blacks .
	manualset3
83699	4	398109	5	NULL	NULL	NULL	NULL	rhesus blood group	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	HLA is the most informative system in all three populations , followed by PGM1 , with the rhesus blood group the next most useful in the whites and ` coloured 's , whereas ABO is the next most useful in the blacks .
	manualset3
83700	5	398109	5	NULL	NULL	NULL	NULL	whites and ` coloured 's	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	HLA is the most informative system in all three populations , followed by PGM1 , with the rhesus blood group the next most useful in the whites and ` coloured 's , whereas ABO is the next most useful in the blacks .
	manualset3
83701	6	398109	5	NULL	NULL	NULL	NULL	ABO	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	HLA is the most informative system in all three populations , followed by PGM1 , with the rhesus blood group the next most useful in the whites and ` coloured 's , whereas ABO is the next most useful in the blacks .
	manualset3
83702	7	398109	5	NULL	NULL	NULL	NULL	blacks	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	HLA is the most informative system in all three populations , followed by PGM1 , with the rhesus blood group the next most useful in the whites and ` coloured 's , whereas ABO is the next most useful in the blacks .
	manualset3
83703	1	398110	5	NULL	NULL	0	NULL	HMGB1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	HMGB1 interacts with human topoisomerase IIalpha and stimulates its catalytic activity .
	manualset3
83704	2	398110	5	NULL	NULL	0	NULL	human topoisomerase IIalpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	HMGB1 interacts with human topoisomerase IIalpha and stimulates its catalytic activity .
	manualset3
83705	3	398110	5	NULL	NULL	0	NULL	catalytic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HMGB1 interacts with human topoisomerase IIalpha and stimulates its catalytic activity .
	manualset3
83706	1	398111	5	NULL	NULL	0	NULL	Storage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Storage and blood coagulation in methylcellulose treated rats ) .
	manualset3
83707	2	398111	5	NULL	NULL	0	NULL	blood coagulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Storage and blood coagulation in methylcellulose treated rats ) .
	manualset3
83708	3	398111	5	NULL	NULL	0	NULL	methylcellulose treated rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Storage and blood coagulation in methylcellulose treated rats ) .
	manualset3
83709	1	398112	5	NULL	NULL	0	NULL	HNa	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	HNa or LNa significantly increased or decreased MAP but had no effects on resting RSNA in SHR and had no effects on resting MAP and RSNA in WKY rats .
	manualset3
83710	2	398112	5	NULL	NULL	0	NULL	LNa	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	HNa or LNa significantly increased or decreased MAP but had no effects on resting RSNA in SHR and had no effects on resting MAP and RSNA in WKY rats .
	manualset3
83711	3	398112	5	NULL	NULL	0	NULL	MAP	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	HNa or LNa significantly increased or decreased MAP but had no effects on resting RSNA in SHR and had no effects on resting MAP and RSNA in WKY rats .
	manualset3
83712	4	398112	5	NULL	NULL	0	NULL	resting RSNA	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HNa or LNa significantly increased or decreased MAP but had no effects on resting RSNA in SHR and had no effects on resting MAP and RSNA in WKY rats .
	manualset3
83713	5	398112	5	NULL	NULL	0	NULL	SHR	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	HNa or LNa significantly increased or decreased MAP but had no effects on resting RSNA in SHR and had no effects on resting MAP and RSNA in WKY rats .
	manualset3
83714	6	398112	5	NULL	NULL	0	NULL	resting MAP	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	HNa or LNa significantly increased or decreased MAP but had no effects on resting RSNA in SHR and had no effects on resting MAP and RSNA in WKY rats .
	manualset3
83715	7	398112	5	NULL	NULL	0	NULL	RSNA	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HNa or LNa significantly increased or decreased MAP but had no effects on resting RSNA in SHR and had no effects on resting MAP and RSNA in WKY rats .
	manualset3
83716	8	398112	5	NULL	NULL	0	NULL	WKY rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	HNa or LNa significantly increased or decreased MAP but had no effects on resting RSNA in SHR and had no effects on resting MAP and RSNA in WKY rats .
	manualset3
83717	1	398113	5	NULL	NULL	0	NULL	HPV 16 and 18 DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	HPV 16 and 18 DNA and virus-encoded antigens , L1 and E6 were found highly prevalent in these cervical carcinomas .
	manualset3
83718	2	398113	5	NULL	NULL	NULL	NULL	virus-encoded antigens , L1 and E6 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	HPV 16 and 18 DNA and virus-encoded antigens , L1 and E6 were found highly prevalent in these cervical carcinomas .
	manualset3
83719	3	398113	5	NULL	NULL	0	NULL	cervical carcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	HPV 16 and 18 DNA and virus-encoded antigens , L1 and E6 were found highly prevalent in these cervical carcinomas .
	manualset3
83720	1	398114	5	NULL	NULL	0	NULL	HPV infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	HPV infections are transient but on average last for more than one year suggesting that HPV has developed means to evade host immunity .
	manualset3
83721	2	398114	5	NULL	NULL	0	NULL	one year	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	HPV infections are transient but on average last for more than one year suggesting that HPV has developed means to evade host immunity .
	manualset3
83722	3	398114	5	NULL	NULL	0	NULL	HPV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	HPV infections are transient but on average last for more than one year suggesting that HPV has developed means to evade host immunity .
	manualset3
83723	4	398114	5	NULL	NULL	0	NULL	host immunity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HPV infections are transient but on average last for more than one year suggesting that HPV has developed means to evade host immunity .
	manualset3
83724	1	398115	5	NULL	NULL	NULL	NULL	HSV-1 antigen	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	HSV-1 antigen , glycoprotein D ( gD ) and regulatory protein ICP27 were detected in 8-18 % of the hypodiploid fraction of PHA-stimulated , HSV-1-infected lymphocytes .
	manualset3
83725	2	398115	5	NULL	NULL	0	NULL	glycoprotein D ( gD )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	HSV-1 antigen , glycoprotein D ( gD ) and regulatory protein ICP27 were detected in 8-18 % of the hypodiploid fraction of PHA-stimulated , HSV-1-infected lymphocytes .
	manualset3
83726	3	398115	5	NULL	NULL	0	NULL	regulatory protein ICP27	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	HSV-1 antigen , glycoprotein D ( gD ) and regulatory protein ICP27 were detected in 8-18 % of the hypodiploid fraction of PHA-stimulated , HSV-1-infected lymphocytes .
	manualset3
83727	4	398115	5	NULL	NULL	0	NULL	8-18 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	HSV-1 antigen , glycoprotein D ( gD ) and regulatory protein ICP27 were detected in 8-18 % of the hypodiploid fraction of PHA-stimulated , HSV-1-infected lymphocytes .
	manualset3
83728	5	398115	5	NULL	NULL	0	NULL	hypodiploid fraction	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	HSV-1 antigen , glycoprotein D ( gD ) and regulatory protein ICP27 were detected in 8-18 % of the hypodiploid fraction of PHA-stimulated , HSV-1-infected lymphocytes .
	manualset3
83729	6	398115	5	NULL	NULL	0	NULL	PHA-stimulated , HSV-1-infected lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	HSV-1 antigen , glycoprotein D ( gD ) and regulatory protein ICP27 were detected in 8-18 % of the hypodiploid fraction of PHA-stimulated , HSV-1-infected lymphocytes .
	manualset3
83730	1	398116	5	NULL	NULL	0	NULL	HSV-2 positive individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	HSV-2 positive individuals were found seropositive to HSV-1 in approximately 95 % of the cases .
	manualset3
83731	2	398116	5	NULL	NULL	0	NULL	HSV-1	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	HSV-2 positive individuals were found seropositive to HSV-1 in approximately 95 % of the cases .
	manualset3
83732	3	398116	5	NULL	NULL	0	NULL	95 % of the cases	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	HSV-2 positive individuals were found seropositive to HSV-1 in approximately 95 % of the cases .
	manualset3
83733	1	398117	5	NULL	NULL	0	NULL	HTP N-oxide ( HTPNO )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	HTP N-oxide ( HTPNO ) exhibits a relatively weak effect on DA uptake .
	manualset3
83734	3	398117	5	NULL	NULL	NULL	NULL	DA uptake	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	HTP N-oxide ( HTPNO ) exhibits a relatively weak effect on DA uptake .
	manualset3
83735	2	398117	5	NULL	NULL	0	NULL	weak effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	HTP N-oxide ( HTPNO ) exhibits a relatively weak effect on DA uptake .
	manualset3
83736	1	398118	5	NULL	NULL	0	NULL	HVC	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	HVC receives new neurons in adulthood .
	manualset3
83737	2	398118	5	NULL	NULL	0	NULL	new neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	HVC receives new neurons in adulthood .
	manualset3
83738	3	398118	5	NULL	NULL	0	NULL	adulthood	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	HVC receives new neurons in adulthood .
	manualset3
83739	1	398119	5	NULL	NULL	0	NULL	Mycobacterium paratuberculosis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Strain of Mycobacterium paratuberculosis ; observations on its isolation and on its pathogenic activity ) .
	manualset3
83740	2	398119	5	NULL	NULL	0	NULL	observations	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Strain of Mycobacterium paratuberculosis ; observations on its isolation and on its pathogenic activity ) .
	manualset3
83741	3	398119	5	NULL	NULL	NULL	NULL	isolation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Strain of Mycobacterium paratuberculosis ; observations on its isolation and on its pathogenic activity ) .
	manualset3
83742	4	398119	5	NULL	NULL	0	NULL	pathogenic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Strain of Mycobacterium paratuberculosis ; observations on its isolation and on its pathogenic activity ) .
	manualset3
83743	1	398120	5	NULL	NULL	0	NULL	HYAL-1 ( hyaluronoglucosaminidase-1 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	HYAL-1 ( hyaluronoglucosaminidase-1 ) belongs to the hyaluronidase family of enzymes that degrade hyaluronic acid .
	manualset3
83744	2	398120	5	NULL	NULL	0	NULL	hyaluronidase family	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	HYAL-1 ( hyaluronoglucosaminidase-1 ) belongs to the hyaluronidase family of enzymes that degrade hyaluronic acid .
	manualset3
83745	3	398120	5	NULL	NULL	0	NULL	enzymes	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	HYAL-1 ( hyaluronoglucosaminidase-1 ) belongs to the hyaluronidase family of enzymes that degrade hyaluronic acid .
	manualset3
83746	4	398120	5	NULL	NULL	0	NULL	hyaluronic acid	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	HYAL-1 ( hyaluronoglucosaminidase-1 ) belongs to the hyaluronidase family of enzymes that degrade hyaluronic acid .
	manualset3
83747	1	398121	5	NULL	NULL	0	NULL	Habitat associations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Habitat associations , reproduction and diet of the Guinean tilapia Tilapia guineensis of the Gambia River floodplains .
	manualset3
83748	2	398121	5	NULL	NULL	0	NULL	reproduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Habitat associations , reproduction and diet of the Guinean tilapia Tilapia guineensis of the Gambia River floodplains .
	manualset3
83749	3	398121	5	NULL	NULL	0	NULL	diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Habitat associations , reproduction and diet of the Guinean tilapia Tilapia guineensis of the Gambia River floodplains .
	manualset3
83750	4	398121	5	NULL	NULL	0	NULL	Guinean tilapia Tilapia guineensis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Habitat associations , reproduction and diet of the Guinean tilapia Tilapia guineensis of the Gambia River floodplains .
	manualset3
83751	5	398121	5	NULL	NULL	0	NULL	Gambia River floodplains	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Habitat associations , reproduction and diet of the Guinean tilapia Tilapia guineensis of the Gambia River floodplains .
	manualset3
83752	1	398122	5	NULL	NULL	0	NULL	Haemangiosarcoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Haemangiosarcoma was diagnosed on biopsy .
	manualset3
83753	2	398122	5	NULL	NULL	0	NULL	biopsy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Haemangiosarcoma was diagnosed on biopsy .
	manualset3
83754	1	398123	5	NULL	NULL	0	NULL	Haematological toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Haematological toxicity was common ( about 40 % of the children , 11 in the twice - and 19 in the once-daily group ) but never severe .
	manualset3
83755	2	398123	5	NULL	NULL	0	NULL	 40 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Haematological toxicity was common ( about 40 % of the children , 11 in the twice - and 19 in the once-daily group ) but never severe .
	manualset3
83756	3	398123	5	NULL	NULL	0	NULL	 children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Haematological toxicity was common ( about 40 % of the children , 11 in the twice - and 19 in the once-daily group ) but never severe .
	manualset3
83757	4	398123	5	NULL	NULL	0	NULL	11 in the twice - and 19 in the once-daily group	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Haematological toxicity was common ( about 40 % of the children , 11 in the twice - and 19 in the once-daily group ) but never severe .
	manualset3
83758	1	398124	5	NULL	NULL	0	NULL	Haemocyte lysate	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Haemocyte lysate was able to activate the plasma proPO indicating location of the prophenoloxidase activating enzyme ( PPAE ) in hemocytes .
	manualset3
83759	2	398124	5	NULL	NULL	0	NULL	plasma proPO	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Haemocyte lysate was able to activate the plasma proPO indicating location of the prophenoloxidase activating enzyme ( PPAE ) in hemocytes .
	manualset3
83760	3	398124	5	NULL	NULL	0	NULL	 prophenoloxidase activating enzyme ( PPAE )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Haemocyte lysate was able to activate the plasma proPO indicating location of the prophenoloxidase activating enzyme ( PPAE ) in hemocytes .
	manualset3
83761	4	398124	5	NULL	NULL	0	NULL	hemocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Haemocyte lysate was able to activate the plasma proPO indicating location of the prophenoloxidase activating enzyme ( PPAE ) in hemocytes .
	manualset3
83762	1	398125	5	NULL	NULL	0	NULL	Haemodynamic changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Haemodynamic changes following carotid occlusion : MRI angiography and transcranial Doppler patterns .
	manualset3
83763	2	398125	5	NULL	NULL	0	NULL	carotid occlusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Haemodynamic changes following carotid occlusion : MRI angiography and transcranial Doppler patterns .
	manualset3
83764	3	398125	5	NULL	NULL	0	NULL	MRI angiography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Haemodynamic changes following carotid occlusion : MRI angiography and transcranial Doppler patterns .
	manualset3
83765	4	398125	5	NULL	NULL	0	NULL	transcranial Doppler patterns	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Haemodynamic changes following carotid occlusion : MRI angiography and transcranial Doppler patterns .
	manualset3
83766	1	398126	5	NULL	NULL	0	NULL	Haemodynamics	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Haemodynamics in early essential hypertension -- still an area of controversy .
	manualset3
83767	2	398126	5	NULL	NULL	0	NULL	early essential hypertension	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Haemodynamics in early essential hypertension -- still an area of controversy .
	manualset3
83768	1	398127	5	NULL	NULL	0	NULL	Haemolytic assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Haemolytic assays were conducted to investigate the activation of the human serum complement system via the classical and alternative pathways .
	manualset3
83769	2	398127	5	NULL	NULL	0	NULL	activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Haemolytic assays were conducted to investigate the activation of the human serum complement system via the classical and alternative pathways .
	manualset3
83770	3	398127	5	NULL	NULL	0	NULL	human serum complement system	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Haemolytic assays were conducted to investigate the activation of the human serum complement system via the classical and alternative pathways .
	manualset3
83771	4	398127	5	NULL	NULL	0	NULL	classical and alternative pathways	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Haemolytic assays were conducted to investigate the activation of the human serum complement system via the classical and alternative pathways .
	manualset3
83772	1	398128	5	NULL	NULL	0	NULL	Haemophilus aphrophilus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Haemophilus aphrophilus isolated from blood .
	manualset3
83773	2	398128	5	NULL	NULL	0	NULL	blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Haemophilus aphrophilus isolated from blood .
	manualset3
83775	1	398130	5	NULL	NULL	0	NULL	Haemorrhagic thrombocythemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Haemorrhagic thrombocythemia : a clinical and laboratory study .
	manualset3
83776	2	398130	5	NULL	NULL	0	NULL	clinical and laboratory study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Haemorrhagic thrombocythemia : a clinical and laboratory study .
	manualset3
83778	1	398131	5	NULL	NULL	0	NULL	Haghighi S	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Haghighi S , Lekman A , Nilsson S , Blomqvist M , Andersen O. Myelin glycosphingolipid immunoreactivity and CSF levels in multiple sclerosis .
	manualset3
83779	2	398131	5	NULL	NULL	0	NULL	Lekman A	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Haghighi S , Lekman A , Nilsson S , Blomqvist M , Andersen O. Myelin glycosphingolipid immunoreactivity and CSF levels in multiple sclerosis .
	manualset3
83780	3	398131	5	NULL	NULL	0	NULL	Nilsson S	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Haghighi S , Lekman A , Nilsson S , Blomqvist M , Andersen O. Myelin glycosphingolipid immunoreactivity and CSF levels in multiple sclerosis .
	manualset3
83781	4	398131	5	NULL	NULL	0	NULL	Blomqvist M	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Haghighi S , Lekman A , Nilsson S , Blomqvist M , Andersen O. Myelin glycosphingolipid immunoreactivity and CSF levels in multiple sclerosis .
	manualset3
83782	5	398131	5	NULL	NULL	0	NULL	Andersen O	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Haghighi S , Lekman A , Nilsson S , Blomqvist M , Andersen O. Myelin glycosphingolipid immunoreactivity and CSF levels in multiple sclerosis .
	manualset3
83783	6	398131	5	NULL	NULL	0	NULL	Myelin glycosphingolipid immunoreactivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Haghighi S , Lekman A , Nilsson S , Blomqvist M , Andersen O. Myelin glycosphingolipid immunoreactivity and CSF levels in multiple sclerosis .
	manualset3
83784	7	398131	5	NULL	NULL	0	NULL	CSF levels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Haghighi S , Lekman A , Nilsson S , Blomqvist M , Andersen O. Myelin glycosphingolipid immunoreactivity and CSF levels in multiple sclerosis .
	manualset3
83785	8	398131	5	NULL	NULL	0	NULL	multiple sclerosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Haghighi S , Lekman A , Nilsson S , Blomqvist M , Andersen O. Myelin glycosphingolipid immunoreactivity and CSF levels in multiple sclerosis .
	manualset3
83786	1	398132	5	NULL	NULL	0	NULL	Hair follicle delivery systems	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hair follicle delivery systems are described , such as liposomes and viral vectors for gene therapy .
	manualset3
83787	2	398132	5	NULL	NULL	NULL	NULL	liposomes	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hair follicle delivery systems are described , such as liposomes and viral vectors for gene therapy .
	manualset3
83788	3	398132	5	NULL	NULL	0	NULL	viral vectors	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Hair follicle delivery systems are described , such as liposomes and viral vectors for gene therapy .
	manualset3
83789	4	398132	5	NULL	NULL	0	NULL	gene therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hair follicle delivery systems are described , such as liposomes and viral vectors for gene therapy .
	manualset3
83790	1	398133	5	NULL	NULL	0	NULL	Hair follicles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Hair follicles : kinetic concepts and human disease .
	manualset3
83791	2	398133	5	NULL	NULL	0	NULL	kinetic concepts	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hair follicles : kinetic concepts and human disease .
	manualset3
83792	3	398133	5	NULL	NULL	0	NULL	human disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hair follicles : kinetic concepts and human disease .
	manualset3
83793	1	398134	5	NULL	NULL	0	NULL	Hair pellets	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Hair pellets of 10 New Zealand rabbits were prepared and shaped as 1 x 1 x 1-cm cubes with the help of fibrin sealant , then inserted subcutaneously .
	manualset3
83794	2	398134	5	NULL	NULL	0	NULL	10 New Zealand rabbits	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hair pellets of 10 New Zealand rabbits were prepared and shaped as 1 x 1 x 1-cm cubes with the help of fibrin sealant , then inserted subcutaneously .
	manualset3
83795	3	398134	5	NULL	NULL	0	NULL	1 x 1 x 1-cm cubes	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Hair pellets of 10 New Zealand rabbits were prepared and shaped as 1 x 1 x 1-cm cubes with the help of fibrin sealant , then inserted subcutaneously .
	manualset3
83796	4	398134	5	NULL	NULL	0	NULL	fibrin sealant	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Hair pellets of 10 New Zealand rabbits were prepared and shaped as 1 x 1 x 1-cm cubes with the help of fibrin sealant , then inserted subcutaneously .
	manualset3
83797	1	398135	5	NULL	NULL	0	NULL	Hairy cell leukemia hemopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hairy cell leukemia hemopathy is a rare lymphod hemopathy type B. 8 cases are reported and diagnosed at Hpital Aziza Othmana over a period of 20 years between 1979 and 1999 , 7 men and one women .
	manualset3
83798	2	398135	5	NULL	NULL	0	NULL	 rare lymphod hemopathy type B	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hairy cell leukemia hemopathy is a rare lymphod hemopathy type B. 8 cases are reported and diagnosed at Hpital Aziza Othmana over a period of 20 years between 1979 and 1999 , 7 men and one women .
	manualset3
83799	3	398135	5	NULL	NULL	NULL	NULL	8 cases	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hairy cell leukemia hemopathy is a rare lymphod hemopathy type B. 8 cases are reported and diagnosed at Hpital Aziza Othmana over a period of 20 years between 1979 and 1999 , 7 men and one women .
	manualset3
83800	4	398135	5	NULL	NULL	0	NULL	Hpital Aziza Othmana	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Hairy cell leukemia hemopathy is a rare lymphod hemopathy type B. 8 cases are reported and diagnosed at Hpital Aziza Othmana over a period of 20 years between 1979 and 1999 , 7 men and one women .
	manualset3
83801	5	398135	5	NULL	NULL	NULL	NULL	20 years	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hairy cell leukemia hemopathy is a rare lymphod hemopathy type B. 8 cases are reported and diagnosed at Hpital Aziza Othmana over a period of 20 years between 1979 and 1999 , 7 men and one women .
	manualset3
83802	7	398135	5	NULL	NULL	NULL	NULL	7 men	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hairy cell leukemia hemopathy is a rare lymphod hemopathy type B. 8 cases are reported and diagnosed at Hpital Aziza Othmana over a period of 20 years between 1979 and 1999 , 7 men and one women .
	manualset3
83803	8	398135	5	NULL	NULL	NULL	NULL	one women	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hairy cell leukemia hemopathy is a rare lymphod hemopathy type B. 8 cases are reported and diagnosed at Hpital Aziza Othmana over a period of 20 years between 1979 and 1999 , 7 men and one women .
	manualset3
84550	6	398135	5	NULL	NULL	0	NULL	between 1979 and 1999	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Hairy cell leukemia hemopathy is a rare lymphod hemopathy type B. 8 cases are reported and diagnosed at Hpital Aziza Othmana over a period of 20 years between 1979 and 1999 , 7 men and one women .
	manualset3
83804	1	398136	5	NULL	NULL	0	NULL	Half of patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Half of patients with IF mutation had a rapid evolution to ESRD , and half recovered .
	manualset3
83805	2	398136	5	NULL	NULL	0	NULL	IF mutation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Half of patients with IF mutation had a rapid evolution to ESRD , and half recovered .
	manualset3
83806	3	398136	5	NULL	NULL	0	NULL	rapid evolution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Half of patients with IF mutation had a rapid evolution to ESRD , and half recovered .
	manualset3
83807	4	398136	5	NULL	NULL	0	NULL	ESRD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Half of patients with IF mutation had a rapid evolution to ESRD , and half recovered .
	manualset3
83808	1	398137	5	NULL	NULL	0	NULL	Structure-activity study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Structure-activity study of the HindIII-I fragment of the L-IVP strain of vaccinia virus genome .
	manualset3
83809	2	398137	5	NULL	NULL	0	NULL	HindIII-I fragment of the L-IVP strain of vaccinia virus genome	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	( Structure-activity study of the HindIII-I fragment of the L-IVP strain of vaccinia virus genome .
	manualset3
83810	1	398138	5	NULL	NULL	0	NULL	 probes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Half of the probes matched , and half did not match , an item in the preceding memory set .
	manualset3
83811	2	398138	5	NULL	NULL	0	NULL	preceding memory set	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Half of the probes matched , and half did not match , an item in the preceding memory set .
	manualset3
83812	1	398139	5	NULL	NULL	0	NULL	Half the groups of experimental and control animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Half the groups of experimental and control animals were also subjected to daily endurance or uphill running exercise to determine the possible preventive effects of exercise .
	manualset3
83813	2	398139	5	NULL	NULL	0	NULL	daily endurance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Half the groups of experimental and control animals were also subjected to daily endurance or uphill running exercise to determine the possible preventive effects of exercise .
	manualset3
83814	3	398139	5	NULL	NULL	0	NULL	uphill running exercise	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Half the groups of experimental and control animals were also subjected to daily endurance or uphill running exercise to determine the possible preventive effects of exercise .
	manualset3
83815	4	398139	5	NULL	NULL	NULL	NULL	 possible preventive effects of exercise	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Half the groups of experimental and control animals were also subjected to daily endurance or uphill running exercise to determine the possible preventive effects of exercise .
	manualset3
83816	1	398140	5	NULL	NULL	0	NULL	monkeys	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Half the monkeys in each group were offered milk ad lib , and half were given restricted quantities .
	manualset3
83817	2	398140	5	NULL	NULL	0	NULL	each group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Half the monkeys in each group were offered milk ad lib , and half were given restricted quantities .
	manualset3
83818	3	398140	5	NULL	NULL	0	NULL	milk ad lib	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Half the monkeys in each group were offered milk ad lib , and half were given restricted quantities .
	manualset3
83819	4	398140	5	NULL	NULL	0	NULL	restricted quantities	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Half the monkeys in each group were offered milk ad lib , and half were given restricted quantities .
	manualset3
83820	1	398141	5	NULL	NULL	0	NULL	Hallux varus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hallux varus : a step-wise approach for correction .
	manualset3
83821	2	398141	5	NULL	NULL	0	NULL	correction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hallux varus : a step-wise approach for correction .
	manualset3
83822	1	398142	5	NULL	NULL	0	NULL	Haloperidol 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Haloperidol , a typical antipsychotic , is the most commonly prescribed medication for the treatment of mental health problems such as agitation and psychosis .
	manualset3
83823	2	398142	5	NULL	NULL	0	NULL	typical antipsychotic	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Haloperidol , a typical antipsychotic , is the most commonly prescribed medication for the treatment of mental health problems such as agitation and psychosis .
	manualset3
83824	3	398142	5	NULL	NULL	0	NULL	most commonly prescribed medication	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Haloperidol , a typical antipsychotic , is the most commonly prescribed medication for the treatment of mental health problems such as agitation and psychosis .
	manualset3
83825	4	398142	5	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Haloperidol , a typical antipsychotic , is the most commonly prescribed medication for the treatment of mental health problems such as agitation and psychosis .
	manualset3
83826	5	398142	5	NULL	NULL	0	NULL	mental health problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Haloperidol , a typical antipsychotic , is the most commonly prescribed medication for the treatment of mental health problems such as agitation and psychosis .
	manualset3
83827	6	398142	5	NULL	NULL	0	NULL	agitation	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Haloperidol , a typical antipsychotic , is the most commonly prescribed medication for the treatment of mental health problems such as agitation and psychosis .
	manualset3
83828	7	398142	5	NULL	NULL	0	NULL	psychosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Haloperidol , a typical antipsychotic , is the most commonly prescribed medication for the treatment of mental health problems such as agitation and psychosis .
	manualset3
83829	1	398143	5	NULL	NULL	0	NULL	Haloperidol catalepsy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Haloperidol catalepsy was increased only by ivc histamine .
	manualset3
83830	2	398143	5	NULL	NULL	0	NULL	ivc histamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Haloperidol catalepsy was increased only by ivc histamine .
	manualset3
83831	1	398144	5	NULL	NULL	0	NULL	Haloperidol 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Haloperidol exerts its therapeutic effects basically by acting on dopamine receptors .
	manualset3
83832	2	398144	5	NULL	NULL	0	NULL	therapeutic effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Haloperidol exerts its therapeutic effects basically by acting on dopamine receptors .
	manualset3
83833	3	398144	5	NULL	NULL	0	NULL	dopamine receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Haloperidol exerts its therapeutic effects basically by acting on dopamine receptors .
	manualset3
83834	1	398145	5	NULL	NULL	0	NULL	Haloperidol treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Haloperidol treatment significantly increased dyskinetic movements and striatal dopamine D2 receptor density compared with controls .
	manualset3
83835	2	398145	5	NULL	NULL	NULL	NULL	dyskinetic movements	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Haloperidol treatment significantly increased dyskinetic movements and striatal dopamine D2 receptor density compared with controls .
	manualset3
83836	3	398145	5	NULL	NULL	0	NULL	striatal dopamine D2 receptor density	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Haloperidol treatment significantly increased dyskinetic movements and striatal dopamine D2 receptor density compared with controls .
	manualset3
83837	4	398145	5	NULL	NULL	0	NULL	controls	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Haloperidol treatment significantly increased dyskinetic movements and striatal dopamine D2 receptor density compared with controls .
	manualset3
83838	1	398146	5	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies of pregnanediol in urine .
	manualset3
83839	2	398146	5	NULL	NULL	0	NULL	pregnanediol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies of pregnanediol in urine .
	manualset3
83840	3	398146	5	NULL	NULL	0	NULL	urine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies of pregnanediol in urine .
	manualset3
83841	1	398147	5	NULL	NULL	NULL	NULL	Hamartoma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hamartoma of the mitral valve with blood cysts : a rare tumor detected by echocardiography .
	manualset3
83842	2	398147	5	NULL	NULL	0	NULL	mitral valve	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Hamartoma of the mitral valve with blood cysts : a rare tumor detected by echocardiography .
	manualset3
83843	3	398147	5	NULL	NULL	0	NULL	blood cysts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hamartoma of the mitral valve with blood cysts : a rare tumor detected by echocardiography .
	manualset3
83844	4	398147	5	NULL	NULL	0	NULL	rare tumor	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hamartoma of the mitral valve with blood cysts : a rare tumor detected by echocardiography .
	manualset3
83845	5	398147	5	NULL	NULL	0	NULL	echocardiography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hamartoma of the mitral valve with blood cysts : a rare tumor detected by echocardiography .
	manualset3
83846	1	398148	5	NULL	NULL	0	NULL	Hamycin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hamycin incorporated into liposomes containing phosphatidylcholine ( SPC ) and phosphatidic acid ( PA ) had reduced toxicity and an enhanced antifungal activity in experimental aspergillosis in balb/c mice .
	manualset3
83847	2	398148	5	NULL	NULL	NULL	NULL	liposomes	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hamycin incorporated into liposomes containing phosphatidylcholine ( SPC ) and phosphatidic acid ( PA ) had reduced toxicity and an enhanced antifungal activity in experimental aspergillosis in balb/c mice .
	manualset3
83848	5	398148	5	NULL	NULL	NULL	NULL	 reduced toxicity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hamycin incorporated into liposomes containing phosphatidylcholine ( SPC ) and phosphatidic acid ( PA ) had reduced toxicity and an enhanced antifungal activity in experimental aspergillosis in balb/c mice .
	manualset3
83849	6	398148	5	NULL	NULL	NULL	NULL	enhanced antifungal activity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hamycin incorporated into liposomes containing phosphatidylcholine ( SPC ) and phosphatidic acid ( PA ) had reduced toxicity and an enhanced antifungal activity in experimental aspergillosis in balb/c mice .
	manualset3
83850	7	398148	5	NULL	NULL	NULL	NULL	experimental aspergillosis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hamycin incorporated into liposomes containing phosphatidylcholine ( SPC ) and phosphatidic acid ( PA ) had reduced toxicity and an enhanced antifungal activity in experimental aspergillosis in balb/c mice .
	manualset3
83851	8	398148	5	NULL	NULL	NULL	NULL	balb/c mice	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hamycin incorporated into liposomes containing phosphatidylcholine ( SPC ) and phosphatidic acid ( PA ) had reduced toxicity and an enhanced antifungal activity in experimental aspergillosis in balb/c mice .
	manualset3
84501	3	398148	5	NULL	NULL	0	NULL	phosphatidylcholine ( SPC )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hamycin incorporated into liposomes containing phosphatidylcholine ( SPC ) and phosphatidic acid ( PA ) had reduced toxicity and an enhanced antifungal activity in experimental aspergillosis in balb/c mice .
	manualset3
84502	4	398148	5	NULL	NULL	0	NULL	phosphatidic acid ( PA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hamycin incorporated into liposomes containing phosphatidylcholine ( SPC ) and phosphatidic acid ( PA ) had reduced toxicity and an enhanced antifungal activity in experimental aspergillosis in balb/c mice .
	manualset3
83852	1	398149	5	NULL	NULL	0	NULL	Hand et al	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hand et al. argued for the importance of including launch site in analyses of target word fixation durations .
	manualset3
83853	2	398149	5	NULL	NULL	0	NULL	launch site	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Hand et al. argued for the importance of including launch site in analyses of target word fixation durations .
	manualset3
83854	3	398149	5	NULL	NULL	0	NULL	target word fixation durations	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Hand et al. argued for the importance of including launch site in analyses of target word fixation durations .
	manualset3
83855	1	398150	5	NULL	NULL	0	NULL	Hand volume	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hand volume , GS ( J ) , GS ( C ) and PS of the dominant hand were respectively 3.6 + / - 4.1 % , 6.6 + / - 9.2 % , 11.7 + / - 11.2 % , and 8.0 + / - 13.2 % higher than those of the non-dominant hand ( p & lt ; 0.001 ) .
	manualset3
83856	2	398150	5	NULL	NULL	0	NULL	GS ( J )	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hand volume , GS ( J ) , GS ( C ) and PS of the dominant hand were respectively 3.6 + / - 4.1 % , 6.6 + / - 9.2 % , 11.7 + / - 11.2 % , and 8.0 + / - 13.2 % higher than those of the non-dominant hand ( p & lt ; 0.001 ) .
	manualset3
83857	3	398150	5	NULL	NULL	0	NULL	GS ( C )	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hand volume , GS ( J ) , GS ( C ) and PS of the dominant hand were respectively 3.6 + / - 4.1 % , 6.6 + / - 9.2 % , 11.7 + / - 11.2 % , and 8.0 + / - 13.2 % higher than those of the non-dominant hand ( p & lt ; 0.001 ) .
	manualset3
83858	4	398150	5	NULL	NULL	0	NULL	PS	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hand volume , GS ( J ) , GS ( C ) and PS of the dominant hand were respectively 3.6 + / - 4.1 % , 6.6 + / - 9.2 % , 11.7 + / - 11.2 % , and 8.0 + / - 13.2 % higher than those of the non-dominant hand ( p & lt ; 0.001 ) .
	manualset3
83859	5	398150	5	NULL	NULL	0	NULL	dominant hand	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Hand volume , GS ( J ) , GS ( C ) and PS of the dominant hand were respectively 3.6 + / - 4.1 % , 6.6 + / - 9.2 % , 11.7 + / - 11.2 % , and 8.0 + / - 13.2 % higher than those of the non-dominant hand ( p & lt ; 0.001 ) .
	manualset3
83860	6	398150	5	NULL	NULL	0	NULL	3.6 + / - 4.1 % , 6.6 + / - 9.2 % , 11.7 + / - 11.2 % , and 8.0 + / - 13.2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Hand volume , GS ( J ) , GS ( C ) and PS of the dominant hand were respectively 3.6 + / - 4.1 % , 6.6 + / - 9.2 % , 11.7 + / - 11.2 % , and 8.0 + / - 13.2 % higher than those of the non-dominant hand ( p & lt ; 0.001 ) .
	manualset3
83861	7	398150	5	NULL	NULL	0	NULL	non-dominant hand	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Hand volume , GS ( J ) , GS ( C ) and PS of the dominant hand were respectively 3.6 + / - 4.1 % , 6.6 + / - 9.2 % , 11.7 + / - 11.2 % , and 8.0 + / - 13.2 % higher than those of the non-dominant hand ( p & lt ; 0.001 ) .
	manualset3
83862	8	398150	5	NULL	NULL	0	NULL	p & lt ; 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Hand volume , GS ( J ) , GS ( C ) and PS of the dominant hand were respectively 3.6 + / - 4.1 % , 6.6 + / - 9.2 % , 11.7 + / - 11.2 % , and 8.0 + / - 13.2 % higher than those of the non-dominant hand ( p & lt ; 0.001 ) .
	manualset3
83863	1	398151	5	NULL	NULL	0	NULL	Hangover	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hangover may be related to propensity to develop alcohol use disorders ( AUDs ) .
	manualset3
83864	2	398151	5	NULL	NULL	0	NULL	propensity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hangover may be related to propensity to develop alcohol use disorders ( AUDs ) .
	manualset3
83865	3	398151	5	NULL	NULL	0	NULL	alcohol use disorders ( AUDs )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hangover may be related to propensity to develop alcohol use disorders ( AUDs ) .
	manualset3
83866	1	398152	5	NULL	NULL	0	NULL	Hans Krebs	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Hans Krebs : nineteen nineteen and after .
	manualset3
83867	2	398152	5	NULL	NULL	0	NULL	nineteen nineteen	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Hans Krebs : nineteen nineteen and after .
	manualset3
83868	1	398153	5	NULL	NULL	0	NULL	Hardware schematics	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Hardware schematics , layout files , and software are freely available .
	manualset3
83869	2	398153	5	NULL	NULL	0	NULL	layout files	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Hardware schematics , layout files , and software are freely available .
	manualset3
83870	3	398153	5	NULL	NULL	0	NULL	software	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Hardware schematics , layout files , and software are freely available .
	manualset3
83871	1	398154	5	NULL	NULL	0	NULL	technical difficulties	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Having solved the technical difficulties of bulk manufacture of IgG concentrates for intravenous use , our attention should now be directed towards preventing viral contamination by both modifying the manufacturing processes and screening the donors for evidence of disease .
	manualset3
83872	2	398154	5	NULL	NULL	0	NULL	bulk manufacture	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Having solved the technical difficulties of bulk manufacture of IgG concentrates for intravenous use , our attention should now be directed towards preventing viral contamination by both modifying the manufacturing processes and screening the donors for evidence of disease .
	manualset3
83873	3	398154	5	NULL	NULL	0	NULL	IgG concentrates	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Having solved the technical difficulties of bulk manufacture of IgG concentrates for intravenous use , our attention should now be directed towards preventing viral contamination by both modifying the manufacturing processes and screening the donors for evidence of disease .
	manualset3
83874	4	398154	5	NULL	NULL	0	NULL	attention	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Having solved the technical difficulties of bulk manufacture of IgG concentrates for intravenous use , our attention should now be directed towards preventing viral contamination by both modifying the manufacturing processes and screening the donors for evidence of disease .
	manualset3
83875	5	398154	5	NULL	NULL	0	NULL	viral contamination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Having solved the technical difficulties of bulk manufacture of IgG concentrates for intravenous use , our attention should now be directed towards preventing viral contamination by both modifying the manufacturing processes and screening the donors for evidence of disease .
	manualset3
83876	6	398154	5	NULL	NULL	0	NULL	manufacturing processes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Having solved the technical difficulties of bulk manufacture of IgG concentrates for intravenous use , our attention should now be directed towards preventing viral contamination by both modifying the manufacturing processes and screening the donors for evidence of disease .
	manualset3
83877	7	398154	5	NULL	NULL	0	NULL	donors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Having solved the technical difficulties of bulk manufacture of IgG concentrates for intravenous use , our attention should now be directed towards preventing viral contamination by both modifying the manufacturing processes and screening the donors for evidence of disease .
	manualset3
83878	8	398154	5	NULL	NULL	0	NULL	evidence of disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Having solved the technical difficulties of bulk manufacture of IgG concentrates for intravenous use , our attention should now be directed towards preventing viral contamination by both modifying the manufacturing processes and screening the donors for evidence of disease .
	manualset3
83879	1	398155	5	NULL	NULL	0	NULL	Hazard analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hazard analysis and risk assessment techniques are utilized within many private sector industries and government agencies , including the medical device and pharmaceutical industry , within a structured process to control human injuries and environmental and property damage .
	manualset3
83880	2	398155	5	NULL	NULL	0	NULL	risk assessment techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hazard analysis and risk assessment techniques are utilized within many private sector industries and government agencies , including the medical device and pharmaceutical industry , within a structured process to control human injuries and environmental and property damage .
	manualset3
83881	3	398155	5	NULL	NULL	0	NULL	private sector industries and government agencies	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Hazard analysis and risk assessment techniques are utilized within many private sector industries and government agencies , including the medical device and pharmaceutical industry , within a structured process to control human injuries and environmental and property damage .
	manualset3
83882	4	398155	5	NULL	NULL	0	NULL	medical device	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Hazard analysis and risk assessment techniques are utilized within many private sector industries and government agencies , including the medical device and pharmaceutical industry , within a structured process to control human injuries and environmental and property damage .
	manualset3
83883	5	398155	5	NULL	NULL	0	NULL	pharmaceutical industry	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Hazard analysis and risk assessment techniques are utilized within many private sector industries and government agencies , including the medical device and pharmaceutical industry , within a structured process to control human injuries and environmental and property damage .
	manualset3
83884	6	398155	5	NULL	NULL	0	NULL	structured process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Hazard analysis and risk assessment techniques are utilized within many private sector industries and government agencies , including the medical device and pharmaceutical industry , within a structured process to control human injuries and environmental and property damage .
	manualset3
83885	7	398155	5	NULL	NULL	NULL	NULL	human injuries	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hazard analysis and risk assessment techniques are utilized within many private sector industries and government agencies , including the medical device and pharmaceutical industry , within a structured process to control human injuries and environmental and property damage .
	manualset3
83886	8	398155	5	NULL	NULL	NULL	NULL	 environmental and property damage	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hazard analysis and risk assessment techniques are utilized within many private sector industries and government agencies , including the medical device and pharmaceutical industry , within a structured process to control human injuries and environmental and property damage .
	manualset3
83889	1	398157	5	NULL	NULL	0	NULL	comatose	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	He became comatose , requiring ventilatory support , and exhibited abnormalities of some brainstem reflexes prior to treatment .
	manualset3
83890	2	398157	5	NULL	NULL	0	NULL	ventilatory support	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	He became comatose , requiring ventilatory support , and exhibited abnormalities of some brainstem reflexes prior to treatment .
	manualset3
83891	3	398157	5	NULL	NULL	0	NULL	brainstem reflexes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	He became comatose , requiring ventilatory support , and exhibited abnormalities of some brainstem reflexes prior to treatment .
	manualset3
83892	4	398157	5	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	He became comatose , requiring ventilatory support , and exhibited abnormalities of some brainstem reflexes prior to treatment .
	manualset3
83893	1	398158	5	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on metabolites of baicalin in human urine ) .
	manualset3
83894	2	398158	5	NULL	NULL	0	NULL	metabolites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on metabolites of baicalin in human urine ) .
	manualset3
83895	3	398158	5	NULL	NULL	0	NULL	baicalin	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on metabolites of baicalin in human urine ) .
	manualset3
83896	4	398158	5	NULL	NULL	0	NULL	human urine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on metabolites of baicalin in human urine ) .
	manualset3
83897	1	398159	5	NULL	NULL	0	NULL	four treatment phases	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	He completed four treatment phases : 6 weeks of detraining , 10 weeks of weight lifting , 10 weeks of running , and 10 weeks of weight lifting .
	manualset3
83898	2	398159	5	NULL	NULL	0	NULL	6 weeks of detraining	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	He completed four treatment phases : 6 weeks of detraining , 10 weeks of weight lifting , 10 weeks of running , and 10 weeks of weight lifting .
	manualset3
83899	3	398159	5	NULL	NULL	0	NULL	10 weeks of weight lifting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	He completed four treatment phases : 6 weeks of detraining , 10 weeks of weight lifting , 10 weeks of running , and 10 weeks of weight lifting .
	manualset3
83900	4	398159	5	NULL	NULL	0	NULL	10 weeks of running	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	He completed four treatment phases : 6 weeks of detraining , 10 weeks of weight lifting , 10 weeks of running , and 10 weeks of weight lifting .
	manualset3
83901	5	398159	5	NULL	NULL	0	NULL	10 weeks of weight lifting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	He completed four treatment phases : 6 weeks of detraining , 10 weeks of weight lifting , 10 weeks of running , and 10 weeks of weight lifting .
	manualset3
83902	1	398160	5	NULL	NULL	0	NULL	explanatory model	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	He devised an explanatory model of this disease , indicating its origin as the variable alteration of the relationship between what he termed thymo and noopsyche .
	manualset3
83903	2	398160	5	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	He devised an explanatory model of this disease , indicating its origin as the variable alteration of the relationship between what he termed thymo and noopsyche .
	manualset3
83904	3	398160	5	NULL	NULL	0	NULL	variable alteration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	He devised an explanatory model of this disease , indicating its origin as the variable alteration of the relationship between what he termed thymo and noopsyche .
	manualset3
83905	4	398160	5	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	He devised an explanatory model of this disease , indicating its origin as the variable alteration of the relationship between what he termed thymo and noopsyche .
	manualset3
83906	5	398160	5	NULL	NULL	NULL	NULL	thymo and noopsyche	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	He devised an explanatory model of this disease , indicating its origin as the variable alteration of the relationship between what he termed thymo and noopsyche .
	manualset3
83907	1	398161	5	NULL	NULL	0	NULL	white forelock	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	He exhibited white forelock , hypopigmented macules and patches , heterochromia irides , and dystopia canthorum .
	manualset3
83908	2	398161	5	NULL	NULL	0	NULL	hypopigmented macules and patches	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	He exhibited white forelock , hypopigmented macules and patches , heterochromia irides , and dystopia canthorum .
	manualset3
83909	3	398161	5	NULL	NULL	0	NULL	heterochromia irides	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	He exhibited white forelock , hypopigmented macules and patches , heterochromia irides , and dystopia canthorum .
	manualset3
83910	4	398161	5	NULL	NULL	0	NULL	dystopia canthorum	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	He exhibited white forelock , hypopigmented macules and patches , heterochromia irides , and dystopia canthorum .
	manualset3
83911	1	398162	5	NULL	NULL	0	NULL	 anti-tumor necrosis factor ( TNF ) alpha therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	He had never received anti-tumor necrosis factor ( TNF ) alpha therapy .
	manualset3
83912	1	398163	5	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on pathophysiological principles of thinking disorders in schizophrenia by means of a motor method with verbal stimuli ) .
	manualset3
83913	2	398163	5	NULL	NULL	0	NULL	pathophysiological principles	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on pathophysiological principles of thinking disorders in schizophrenia by means of a motor method with verbal stimuli ) .
	manualset3
83914	3	398163	5	NULL	NULL	0	NULL	thinking disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on pathophysiological principles of thinking disorders in schizophrenia by means of a motor method with verbal stimuli ) .
	manualset3
83915	4	398163	5	NULL	NULL	0	NULL	schizophrenia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on pathophysiological principles of thinking disorders in schizophrenia by means of a motor method with verbal stimuli ) .
	manualset3
83916	5	398163	5	NULL	NULL	0	NULL	motor method with verbal stimuli	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on pathophysiological principles of thinking disorders in schizophrenia by means of a motor method with verbal stimuli ) .
	manualset3
83917	1	398164	5	NULL	NULL	0	NULL	5 FC ( 5-fluorocytosine ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	He is on 5 FC ( 5-fluorocytosine ) , Minomycin ( minocycline hydrochloride ) , and Baktar ( trimethoprim-sulfamethoxazole ) .
	manualset3
83918	2	398164	5	NULL	NULL	0	NULL	Minomycin ( minocycline hydrochloride ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	He is on 5 FC ( 5-fluorocytosine ) , Minomycin ( minocycline hydrochloride ) , and Baktar ( trimethoprim-sulfamethoxazole ) .
	manualset3
83919	3	398164	5	NULL	NULL	0	NULL	Baktar ( trimethoprim-sulfamethoxazole )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	He is on 5 FC ( 5-fluorocytosine ) , Minomycin ( minocycline hydrochloride ) , and Baktar ( trimethoprim-sulfamethoxazole ) .
	manualset3
84493	1	398165	5	NULL	NULL	0	NULL	recent relevant directions	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	He outlines recent relevant directions of the Joint Commission on Accreditation of Healthcare Organizations , especially the shift to continuous quality improvement and the organization of the 1995 standards around major functions such as improving performance .
	manualset3
84494	2	398165	5	NULL	NULL	0	NULL	Joint Commission	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	He outlines recent relevant directions of the Joint Commission on Accreditation of Healthcare Organizations , especially the shift to continuous quality improvement and the organization of the 1995 standards around major functions such as improving performance .
	manualset3
84495	3	398165	5	NULL	NULL	0	NULL	Accreditation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	He outlines recent relevant directions of the Joint Commission on Accreditation of Healthcare Organizations , especially the shift to continuous quality improvement and the organization of the 1995 standards around major functions such as improving performance .
	manualset3
84496	4	398165	5	NULL	NULL	0	NULL	Healthcare Organizations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	He outlines recent relevant directions of the Joint Commission on Accreditation of Healthcare Organizations , especially the shift to continuous quality improvement and the organization of the 1995 standards around major functions such as improving performance .
	manualset3
84497	5	398165	5	NULL	NULL	0	NULL	continuous quality improvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	He outlines recent relevant directions of the Joint Commission on Accreditation of Healthcare Organizations , especially the shift to continuous quality improvement and the organization of the 1995 standards around major functions such as improving performance .
	manualset3
84498	6	398165	5	NULL	NULL	0	NULL	organization	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	He outlines recent relevant directions of the Joint Commission on Accreditation of Healthcare Organizations , especially the shift to continuous quality improvement and the organization of the 1995 standards around major functions such as improving performance .
	manualset3
84499	7	398165	5	NULL	NULL	0	NULL	1995 standards	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	He outlines recent relevant directions of the Joint Commission on Accreditation of Healthcare Organizations , especially the shift to continuous quality improvement and the organization of the 1995 standards around major functions such as improving performance .
	manualset3
84500	8	398165	5	NULL	NULL	0	NULL	major functions such as improving performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	He outlines recent relevant directions of the Joint Commission on Accreditation of Healthcare Organizations , especially the shift to continuous quality improvement and the organization of the 1995 standards around major functions such as improving performance .
	manualset3
83920	1	398166	5	NULL	NULL	0	NULL	symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	He presented all the symptoms : urethritis , conjunctivitis , arthritis , balanitis circinata and keratodermia .
	manualset3
83921	2	398166	5	NULL	NULL	0	NULL	urethritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	He presented all the symptoms : urethritis , conjunctivitis , arthritis , balanitis circinata and keratodermia .
	manualset3
83922	3	398166	5	NULL	NULL	0	NULL	conjunctivitis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	He presented all the symptoms : urethritis , conjunctivitis , arthritis , balanitis circinata and keratodermia .
	manualset3
83923	4	398166	5	NULL	NULL	0	NULL	arthritis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	He presented all the symptoms : urethritis , conjunctivitis , arthritis , balanitis circinata and keratodermia .
	manualset3
83924	5	398166	5	NULL	NULL	0	NULL	balanitis circinata	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	He presented all the symptoms : urethritis , conjunctivitis , arthritis , balanitis circinata and keratodermia .
	manualset3
83925	6	398166	5	NULL	NULL	0	NULL	keratodermia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	He presented all the symptoms : urethritis , conjunctivitis , arthritis , balanitis circinata and keratodermia .
	manualset3
83926	1	398167	5	NULL	NULL	0	NULL	establishment of psychiatric hospitals	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	He proposed the establishment of psychiatric hospitals in order to eliminate the hospitalization of the sick in the same building as healthy and to permit the application of specific forms of treatment .
	manualset3
83927	2	398167	5	NULL	NULL	0	NULL	hospitalization 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	He proposed the establishment of psychiatric hospitals in order to eliminate the hospitalization of the sick in the same building as healthy and to permit the application of specific forms of treatment .
	manualset3
83928	3	398167	5	NULL	NULL	0	NULL	sick 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	He proposed the establishment of psychiatric hospitals in order to eliminate the hospitalization of the sick in the same building as healthy and to permit the application of specific forms of treatment .
	manualset3
83929	4	398167	5	NULL	NULL	0	NULL	same building	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	He proposed the establishment of psychiatric hospitals in order to eliminate the hospitalization of the sick in the same building as healthy and to permit the application of specific forms of treatment .
	manualset3
83930	5	398167	5	NULL	NULL	NULL	NULL	application	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	He proposed the establishment of psychiatric hospitals in order to eliminate the hospitalization of the sick in the same building as healthy and to permit the application of specific forms of treatment .
	manualset3
83931	6	398167	5	NULL	NULL	0	NULL	specific forms of treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	He proposed the establishment of psychiatric hospitals in order to eliminate the hospitalization of the sick in the same building as healthy and to permit the application of specific forms of treatment .
	manualset3
83932	1	398168	5	NULL	NULL	0	NULL	2 courses of CDDP/TXT chemotherapy ( cisplatin 75 mg/m2 , docetaxel 80 mg/m2 )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	He received 2 courses of CDDP/TXT chemotherapy ( cisplatin 75 mg/m2 , docetaxel 80 mg/m2 ) and achieved a partial response , but his carcinoma of the pancreas recurred .
	manualset3
83933	2	398168	5	NULL	NULL	0	NULL	partial response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	He received 2 courses of CDDP/TXT chemotherapy ( cisplatin 75 mg/m2 , docetaxel 80 mg/m2 ) and achieved a partial response , but his carcinoma of the pancreas recurred .
	manualset3
83934	3	398168	5	NULL	NULL	NULL	NULL	carcinoma of the pancreas	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	He received 2 courses of CDDP/TXT chemotherapy ( cisplatin 75 mg/m2 , docetaxel 80 mg/m2 ) and achieved a partial response , but his carcinoma of the pancreas recurred .
	manualset3
83936	1	398169	5	NULL	NULL	0	NULL	recurrence of a similar episode	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	He recovered completely , but the recurrence of a similar episode with associated cardiomyopathy and dicarboxylic aciduria at 10 months of age led to the recognition of a fatty acid oxidation defect .
	manualset3
83937	2	398169	5	NULL	NULL	0	NULL	associated cardiomyopathy and dicarboxylic aciduria	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	He recovered completely , but the recurrence of a similar episode with associated cardiomyopathy and dicarboxylic aciduria at 10 months of age led to the recognition of a fatty acid oxidation defect .
	manualset3
83938	3	398169	5	NULL	NULL	0	NULL	10 months of age	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	He recovered completely , but the recurrence of a similar episode with associated cardiomyopathy and dicarboxylic aciduria at 10 months of age led to the recognition of a fatty acid oxidation defect .
	manualset3
83939	4	398169	5	NULL	NULL	0	NULL	recognition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	He recovered completely , but the recurrence of a similar episode with associated cardiomyopathy and dicarboxylic aciduria at 10 months of age led to the recognition of a fatty acid oxidation defect .
	manualset3
83940	5	398169	5	NULL	NULL	0	NULL	fatty acid oxidation defect	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	He recovered completely , but the recurrence of a similar episode with associated cardiomyopathy and dicarboxylic aciduria at 10 months of age led to the recognition of a fatty acid oxidation defect .
	manualset3
83941	1	398170	5	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on the causative agent of Hyuga-feveri ; cultivation of rickettsia-like organisms isolated from metacercariae of Stellantchasumus falcatus in tissue culture cell and their antigenic relation to Rickettsia sennetsu ( author 's transl ) ) .
	manualset3
83942	2	398170	5	NULL	NULL	0	NULL	causative agent of Hyuga-feveri	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on the causative agent of Hyuga-feveri ; cultivation of rickettsia-like organisms isolated from metacercariae of Stellantchasumus falcatus in tissue culture cell and their antigenic relation to Rickettsia sennetsu ( author 's transl ) ) .
	manualset3
83943	3	398170	5	NULL	NULL	0	NULL	cultivation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on the causative agent of Hyuga-feveri ; cultivation of rickettsia-like organisms isolated from metacercariae of Stellantchasumus falcatus in tissue culture cell and their antigenic relation to Rickettsia sennetsu ( author 's transl ) ) .
	manualset3
83944	4	398170	5	NULL	NULL	0	NULL	rickettsia-like organisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on the causative agent of Hyuga-feveri ; cultivation of rickettsia-like organisms isolated from metacercariae of Stellantchasumus falcatus in tissue culture cell and their antigenic relation to Rickettsia sennetsu ( author 's transl ) ) .
	manualset3
83945	5	398170	5	NULL	NULL	0	NULL	metacercariae of Stellantchasumus falcatus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on the causative agent of Hyuga-feveri ; cultivation of rickettsia-like organisms isolated from metacercariae of Stellantchasumus falcatus in tissue culture cell and their antigenic relation to Rickettsia sennetsu ( author 's transl ) ) .
	manualset3
83946	6	398170	5	NULL	NULL	0	NULL	tissue culture cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on the causative agent of Hyuga-feveri ; cultivation of rickettsia-like organisms isolated from metacercariae of Stellantchasumus falcatus in tissue culture cell and their antigenic relation to Rickettsia sennetsu ( author 's transl ) ) .
	manualset3
83947	7	398170	5	NULL	NULL	0	NULL	antigenic relation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on the causative agent of Hyuga-feveri ; cultivation of rickettsia-like organisms isolated from metacercariae of Stellantchasumus falcatus in tissue culture cell and their antigenic relation to Rickettsia sennetsu ( author 's transl ) ) .
	manualset3
83948	8	398170	5	NULL	NULL	0	NULL	Rickettsia sennetsu	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on the causative agent of Hyuga-feveri ; cultivation of rickettsia-like organisms isolated from metacercariae of Stellantchasumus falcatus in tissue culture cell and their antigenic relation to Rickettsia sennetsu ( author 's transl ) ) .
	manualset3
83949	1	398171	5	NULL	NULL	NULL	NULL	pontine hemorrhage	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	He subsequently developed a pontine hemorrhage and acute hydrocephalus and died secondary to transtentorial herniation .
	manualset3
83950	2	398171	5	NULL	NULL	0	NULL	acute hydrocephalus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	He subsequently developed a pontine hemorrhage and acute hydrocephalus and died secondary to transtentorial herniation .
	manualset3
83952	4	398171	5	NULL	NULL	NULL	NULL	transtentorial herniation	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	He subsequently developed a pontine hemorrhage and acute hydrocephalus and died secondary to transtentorial herniation .
	manualset3
83953	1	398172	5	NULL	NULL	0	NULL	ethanol intake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	He successfully reduced his ethanol intake over a 3-month period , but he was unable to sustain abstinence .
	manualset3
83954	2	398172	5	NULL	NULL	0	NULL	over a 3-month period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	He successfully reduced his ethanol intake over a 3-month period , but he was unable to sustain abstinence .
	manualset3
83955	3	398172	5	NULL	NULL	0	NULL	sustain abstinence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	He successfully reduced his ethanol intake over a 3-month period , but he was unable to sustain abstinence .
	manualset3
83956	1	398173	5	NULL	NULL	0	NULL	BD with oral ulcer , genital ulcer , papular skin lesion , deep vein thrombosis ( DVT ) and positive pathergy reaction	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	He was diagnosed as having BD with oral ulcer , genital ulcer , papular skin lesion , deep vein thrombosis ( DVT ) and positive pathergy reaction .
	manualset3
83957	1	398174	5	NULL	NULL	0	NULL	heparin-induced thrombocytopenia and thrombosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	He was found to have developed heparin-induced thrombocytopenia and thrombosis , confirmed by high levels of heparin-platelet factor 4-antibody on enzyme-linked immunosorbent assay ( ELISA ) .
	manualset3
83958	2	398174	5	NULL	NULL	0	NULL	high levels of heparin-platelet factor 4-antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	He was found to have developed heparin-induced thrombocytopenia and thrombosis , confirmed by high levels of heparin-platelet factor 4-antibody on enzyme-linked immunosorbent assay ( ELISA ) .
	manualset3
83959	3	398174	5	NULL	NULL	0	NULL	enzyme-linked immunosorbent assay ( ELISA )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	He was found to have developed heparin-induced thrombocytopenia and thrombosis , confirmed by high levels of heparin-platelet factor 4-antibody on enzyme-linked immunosorbent assay ( ELISA ) .
	manualset3
83960	1	398175	5	NULL	NULL	0	NULL	pediatric dentist	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	He was initially evaluated by a pediatric dentist and epidermal dysplasia syndromes were considered , but insensitivity to pain was suspected after a skeletal survey revealed an unrecognized skull fracture .
	manualset3
83961	2	398175	5	NULL	NULL	0	NULL	epidermal dysplasia syndromes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	He was initially evaluated by a pediatric dentist and epidermal dysplasia syndromes were considered , but insensitivity to pain was suspected after a skeletal survey revealed an unrecognized skull fracture .
	manualset3
83962	3	398175	5	NULL	NULL	0	NULL	insensitivity to pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	He was initially evaluated by a pediatric dentist and epidermal dysplasia syndromes were considered , but insensitivity to pain was suspected after a skeletal survey revealed an unrecognized skull fracture .
	manualset3
83963	4	398175	5	NULL	NULL	0	NULL	skeletal survey	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	He was initially evaluated by a pediatric dentist and epidermal dysplasia syndromes were considered , but insensitivity to pain was suspected after a skeletal survey revealed an unrecognized skull fracture .
	manualset3
83964	5	398175	5	NULL	NULL	0	NULL	 unrecognized skull fracture	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	He was initially evaluated by a pediatric dentist and epidermal dysplasia syndromes were considered , but insensitivity to pain was suspected after a skeletal survey revealed an unrecognized skull fracture .
	manualset3
83965	1	398176	5	NULL	NULL	0	NULL	pretreated	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	He was pretreated with 300 mg of aspirin , 600 mg of clopidogrel , and was taken to the catheterization laboratory .
	manualset3
83966	2	398176	5	NULL	NULL	0	NULL	 300 mg of aspirin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	He was pretreated with 300 mg of aspirin , 600 mg of clopidogrel , and was taken to the catheterization laboratory .
	manualset3
83967	3	398176	5	NULL	NULL	0	NULL	600 mg of clopidogrel	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	He was pretreated with 300 mg of aspirin , 600 mg of clopidogrel , and was taken to the catheterization laboratory .
	manualset3
83968	4	398176	5	NULL	NULL	0	NULL	catheterization laboratory	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	He was pretreated with 300 mg of aspirin , 600 mg of clopidogrel , and was taken to the catheterization laboratory .
	manualset3
83969	1	398177	5	NULL	NULL	0	NULL	chemotherapy ( CHOP )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	He was treated with chemotherapy ( CHOP ) and radiation , and achieved complete remission .
	manualset3
83970	2	398177	5	NULL	NULL	0	NULL	radiation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	He was treated with chemotherapy ( CHOP ) and radiation , and achieved complete remission .
	manualset3
83971	3	398177	5	NULL	NULL	0	NULL	complete remission	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	He was treated with chemotherapy ( CHOP ) and radiation , and achieved complete remission .
	manualset3
83972	1	398178	5	NULL	NULL	0	NULL	Head louse	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Head louse and other common infections in schools : head teachers ' use of an information pack .
	manualset3
83973	2	398178	5	NULL	NULL	0	NULL	other common infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Head louse and other common infections in schools : head teachers ' use of an information pack .
	manualset3
83974	3	398178	5	NULL	NULL	0	NULL	schools	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Head louse and other common infections in schools : head teachers ' use of an information pack .
	manualset3
83975	4	398178	5	NULL	NULL	0	NULL	head teachers '	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Head louse and other common infections in schools : head teachers ' use of an information pack .
	manualset3
83976	5	398178	5	NULL	NULL	0	NULL	information pack	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Head louse and other common infections in schools : head teachers ' use of an information pack .
	manualset3
83977	1	398179	5	NULL	NULL	0	NULL	Health	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Health , illness , and immigration .
	manualset3
83978	2	398179	5	NULL	NULL	0	NULL	illness 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Health , illness , and immigration .
	manualset3
83979	3	398179	5	NULL	NULL	0	NULL	immigration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Health , illness , and immigration .
	manualset3
83980	1	398180	5	NULL	NULL	0	NULL	Health care delivery system	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Health care delivery system in France : effects on surgical education .
	manualset3
83981	2	398180	5	NULL	NULL	0	NULL	France	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Health care delivery system in France : effects on surgical education .
	manualset3
83982	3	398180	5	NULL	NULL	NULL	NULL	surgical education	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Health care delivery system in France : effects on surgical education .
	manualset3
83983	1	398181	5	NULL	NULL	0	NULL	Health care delivery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Health care delivery to homeless youth was often nonanticipatory , inconsistent and perceived as discriminatory .
	manualset3
83984	2	398181	5	NULL	NULL	0	NULL	homeless youth	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Health care delivery to homeless youth was often nonanticipatory , inconsistent and perceived as discriminatory .
	manualset3
83985	1	398182	5	NULL	NULL	0	NULL	Health services research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Health services research comes of age : three new volumes document the history , development , and present state of the field .
	manualset3
83986	2	398182	5	NULL	NULL	0	NULL	age	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Health services research comes of age : three new volumes document the history , development , and present state of the field .
	manualset3
83987	3	398182	5	NULL	NULL	0	NULL	three new volumes document	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Health services research comes of age : three new volumes document the history , development , and present state of the field .
	manualset3
83988	4	398182	5	NULL	NULL	0	NULL	history	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Health services research comes of age : three new volumes document the history , development , and present state of the field .
	manualset3
83989	5	398182	5	NULL	NULL	0	NULL	present state of the field	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Health services research comes of age : three new volumes document the history , development , and present state of the field .
	manualset3
83990	1	398183	5	NULL	NULL	0	NULL	Healthcare organizations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Healthcare organizations must adopt a new paradigm of care that holds patient safety as a core value and practice .
	manualset3
83991	2	398183	5	NULL	NULL	0	NULL	new paradigm of care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Healthcare organizations must adopt a new paradigm of care that holds patient safety as a core value and practice .
	manualset3
83992	3	398183	5	NULL	NULL	0	NULL	holds patient safety	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Healthcare organizations must adopt a new paradigm of care that holds patient safety as a core value and practice .
	manualset3
83993	4	398183	5	NULL	NULL	0	NULL	core value and practice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Healthcare organizations must adopt a new paradigm of care that holds patient safety as a core value and practice .
	manualset3
84211	1	398184	5	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on the formation of antibodies against antigens in protein extracts of psoriatic scales from the patients with psoriatic arthritis ) .
	manualset3
84212	2	398184	5	NULL	NULL	0	NULL	formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on the formation of antibodies against antigens in protein extracts of psoriatic scales from the patients with psoriatic arthritis ) .
	manualset3
84213	3	398184	5	NULL	NULL	0	NULL	antibodies	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on the formation of antibodies against antigens in protein extracts of psoriatic scales from the patients with psoriatic arthritis ) .
	manualset3
84214	4	398184	5	NULL	NULL	0	NULL	antigens	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on the formation of antibodies against antigens in protein extracts of psoriatic scales from the patients with psoriatic arthritis ) .
	manualset3
84215	5	398184	5	NULL	NULL	0	NULL	protein extracts	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on the formation of antibodies against antigens in protein extracts of psoriatic scales from the patients with psoriatic arthritis ) .
	manualset3
84216	6	398184	5	NULL	NULL	0	NULL	psoriatic scales	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on the formation of antibodies against antigens in protein extracts of psoriatic scales from the patients with psoriatic arthritis ) .
	manualset3
84217	7	398184	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on the formation of antibodies against antigens in protein extracts of psoriatic scales from the patients with psoriatic arthritis ) .
	manualset3
84218	8	398184	5	NULL	NULL	0	NULL	psoriatic arthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on the formation of antibodies against antigens in protein extracts of psoriatic scales from the patients with psoriatic arthritis ) .
	manualset3
84219	1	398185	5	NULL	NULL	0	NULL	Healthcare professionals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Healthcare professionals should be aware that not all men ( or women ) conform to the social stereotypes of masculinity ( or femininity ) .
	manualset3
84220	2	398185	5	NULL	NULL	0	NULL	men ( or women )	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Healthcare professionals should be aware that not all men ( or women ) conform to the social stereotypes of masculinity ( or femininity ) .
	manualset3
84221	3	398185	5	NULL	NULL	0	NULL	social stereotypes	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Healthcare professionals should be aware that not all men ( or women ) conform to the social stereotypes of masculinity ( or femininity ) .
	manualset3
84222	4	398185	5	NULL	NULL	0	NULL	masculinity ( or femininity )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Healthcare professionals should be aware that not all men ( or women ) conform to the social stereotypes of masculinity ( or femininity ) .
	manualset3
84223	1	398186	5	NULL	NULL	0	NULL	Healthy vegetarians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Healthy vegetarians ( 12 male , 12 female ) consumed nine capsules daily of either DHA ( 1.62 g/d ) or corn oil for 6 wk .
	manualset3
84224	2	398186	5	NULL	NULL	0	NULL	 ( 12 male , 12 female )	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Healthy vegetarians ( 12 male , 12 female ) consumed nine capsules daily of either DHA ( 1.62 g/d ) or corn oil for 6 wk .
	manualset3
84225	3	398186	5	NULL	NULL	NULL	NULL	nine capsules	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Healthy vegetarians ( 12 male , 12 female ) consumed nine capsules daily of either DHA ( 1.62 g/d ) or corn oil for 6 wk .
	manualset3
84226	4	398186	5	NULL	NULL	0	NULL	DHA ( 1.62 g/d )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Healthy vegetarians ( 12 male , 12 female ) consumed nine capsules daily of either DHA ( 1.62 g/d ) or corn oil for 6 wk .
	manualset3
84227	5	398186	5	NULL	NULL	0	NULL	corn oil	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Healthy vegetarians ( 12 male , 12 female ) consumed nine capsules daily of either DHA ( 1.62 g/d ) or corn oil for 6 wk .
	manualset3
84228	6	398186	5	NULL	NULL	0	NULL	6 wk	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Healthy vegetarians ( 12 male , 12 female ) consumed nine capsules daily of either DHA ( 1.62 g/d ) or corn oil for 6 wk .
	manualset3
84269	1	398187	5	NULL	NULL	0	NULL	Hearing aid benefit	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hearing aid benefit related to the POGO amplification formula , evaluated from insertion gain measurements of two BTE hearing aids .
	manualset3
84270	2	398187	5	NULL	NULL	0	NULL	POGO amplification formula	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Hearing aid benefit related to the POGO amplification formula , evaluated from insertion gain measurements of two BTE hearing aids .
	manualset3
84271	3	398187	5	NULL	NULL	0	NULL	 insertion gain measurements	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hearing aid benefit related to the POGO amplification formula , evaluated from insertion gain measurements of two BTE hearing aids .
	manualset3
84272	4	398187	5	NULL	NULL	0	NULL	two BTE hearing aids	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Hearing aid benefit related to the POGO amplification formula , evaluated from insertion gain measurements of two BTE hearing aids .
	manualset3
84273	1	398188	5	NULL	NULL	0	NULL	Heart rate	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heart rate , oxygen consumption ( VO2 ) , respiratory exchange ratio ( RER ) , and ratings of perceived exertion ( RPE ) were measured during the preload , and blood glucose and lactate were measured before and after the preload and time-trial .
	manualset3
84274	2	398188	5	NULL	NULL	0	NULL	oxygen consumption ( VO2 )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heart rate , oxygen consumption ( VO2 ) , respiratory exchange ratio ( RER ) , and ratings of perceived exertion ( RPE ) were measured during the preload , and blood glucose and lactate were measured before and after the preload and time-trial .
	manualset3
84275	3	398188	5	NULL	NULL	0	NULL	respiratory exchange ratio ( RER )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heart rate , oxygen consumption ( VO2 ) , respiratory exchange ratio ( RER ) , and ratings of perceived exertion ( RPE ) were measured during the preload , and blood glucose and lactate were measured before and after the preload and time-trial .
	manualset3
84276	4	398188	5	NULL	NULL	0	NULL	ratings of perceived exertion ( RPE )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heart rate , oxygen consumption ( VO2 ) , respiratory exchange ratio ( RER ) , and ratings of perceived exertion ( RPE ) were measured during the preload , and blood glucose and lactate were measured before and after the preload and time-trial .
	manualset3
84277	5	398188	5	NULL	NULL	0	NULL	preload	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Heart rate , oxygen consumption ( VO2 ) , respiratory exchange ratio ( RER ) , and ratings of perceived exertion ( RPE ) were measured during the preload , and blood glucose and lactate were measured before and after the preload and time-trial .
	manualset3
84278	6	398188	5	NULL	NULL	0	NULL	blood glucose	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Heart rate , oxygen consumption ( VO2 ) , respiratory exchange ratio ( RER ) , and ratings of perceived exertion ( RPE ) were measured during the preload , and blood glucose and lactate were measured before and after the preload and time-trial .
	manualset3
84279	7	398188	5	NULL	NULL	0	NULL	lactate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Heart rate , oxygen consumption ( VO2 ) , respiratory exchange ratio ( RER ) , and ratings of perceived exertion ( RPE ) were measured during the preload , and blood glucose and lactate were measured before and after the preload and time-trial .
	manualset3
84280	8	398188	5	NULL	NULL	0	NULL	 preload	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Heart rate , oxygen consumption ( VO2 ) , respiratory exchange ratio ( RER ) , and ratings of perceived exertion ( RPE ) were measured during the preload , and blood glucose and lactate were measured before and after the preload and time-trial .
	manualset3
84281	9	398188	5	NULL	NULL	0	NULL	time-trial	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Heart rate , oxygen consumption ( VO2 ) , respiratory exchange ratio ( RER ) , and ratings of perceived exertion ( RPE ) were measured during the preload , and blood glucose and lactate were measured before and after the preload and time-trial .
	manualset3
84282	1	398189	5	NULL	NULL	0	NULL	Heart rate	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heart rate , pupil size , pupillary light reflex , BIS scores , and blood pressure were measured every 2min before and for 30min after drug administration .
	manualset3
84283	2	398189	5	NULL	NULL	0	NULL	pupillary light reflex	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heart rate , pupil size , pupillary light reflex , BIS scores , and blood pressure were measured every 2min before and for 30min after drug administration .
	manualset3
84284	3	398189	5	NULL	NULL	0	NULL	BIS scores	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heart rate , pupil size , pupillary light reflex , BIS scores , and blood pressure were measured every 2min before and for 30min after drug administration .
	manualset3
84285	4	398189	5	NULL	NULL	0	NULL	blood pressure	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heart rate , pupil size , pupillary light reflex , BIS scores , and blood pressure were measured every 2min before and for 30min after drug administration .
	manualset3
84286	5	398189	5	NULL	NULL	0	NULL	2min 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Heart rate , pupil size , pupillary light reflex , BIS scores , and blood pressure were measured every 2min before and for 30min after drug administration .
	manualset3
84287	6	398189	5	NULL	NULL	0	NULL	30min	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Heart rate , pupil size , pupillary light reflex , BIS scores , and blood pressure were measured every 2min before and for 30min after drug administration .
	manualset3
84288	7	398189	5	NULL	NULL	0	NULL	drug administration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heart rate , pupil size , pupillary light reflex , BIS scores , and blood pressure were measured every 2min before and for 30min after drug administration .
	manualset3
84289	1	398190	5	NULL	NULL	0	NULL	Hearts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Hearts of aged animals contained significantly ( P & lt ; 0.05 ; ANOVA ) more proANF 1-98 , proANF 31-67 , and ANF than hearts of adult animals .
	manualset3
84290	2	398190	5	NULL	NULL	0	NULL	aged animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hearts of aged animals contained significantly ( P & lt ; 0.05 ; ANOVA ) more proANF 1-98 , proANF 31-67 , and ANF than hearts of adult animals .
	manualset3
84291	3	398190	5	NULL	NULL	0	NULL	P & lt ; 0.05 ; ANOVA	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Hearts of aged animals contained significantly ( P & lt ; 0.05 ; ANOVA ) more proANF 1-98 , proANF 31-67 , and ANF than hearts of adult animals .
	manualset3
84292	4	398190	5	NULL	NULL	0	NULL	proANF 1-98	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hearts of aged animals contained significantly ( P & lt ; 0.05 ; ANOVA ) more proANF 1-98 , proANF 31-67 , and ANF than hearts of adult animals .
	manualset3
84293	5	398190	5	NULL	NULL	0	NULL	proANF 31-67	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hearts of aged animals contained significantly ( P & lt ; 0.05 ; ANOVA ) more proANF 1-98 , proANF 31-67 , and ANF than hearts of adult animals .
	manualset3
84294	6	398190	5	NULL	NULL	0	NULL	ANF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hearts of aged animals contained significantly ( P & lt ; 0.05 ; ANOVA ) more proANF 1-98 , proANF 31-67 , and ANF than hearts of adult animals .
	manualset3
84295	7	398190	5	NULL	NULL	0	NULL	hearts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Hearts of aged animals contained significantly ( P & lt ; 0.05 ; ANOVA ) more proANF 1-98 , proANF 31-67 , and ANF than hearts of adult animals .
	manualset3
84296	8	398190	5	NULL	NULL	0	NULL	adult animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hearts of aged animals contained significantly ( P & lt ; 0.05 ; ANOVA ) more proANF 1-98 , proANF 31-67 , and ANF than hearts of adult animals .
	manualset3
84297	1	398191	5	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on the mechanism of action of so-called radiation-protective agents and agents against radiation damage ) .
	manualset3
84298	2	398191	5	NULL	NULL	0	NULL	mechanism of action	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on the mechanism of action of so-called radiation-protective agents and agents against radiation damage ) .
	manualset3
84299	3	398191	5	NULL	NULL	0	NULL	radiation-protective agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on the mechanism of action of so-called radiation-protective agents and agents against radiation damage ) .
	manualset3
84300	4	398191	5	NULL	NULL	NULL	NULL	agents against radiation damage	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Studies on the mechanism of action of so-called radiation-protective agents and agents against radiation damage ) .
	manualset3
84301	1	398192	5	NULL	NULL	0	NULL	Hearts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Hearts were removed and mitochondria were isolated .
	manualset3
84302	2	398192	5	NULL	NULL	0	NULL	mitochondria	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Hearts were removed and mitochondria were isolated .
	manualset3
84303	1	398193	5	NULL	NULL	0	NULL	Heat-shock activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat-shock activation of the mutant HNF1B variants P328L329del and A263insGG resulted in malformations of various organs and the affected larvae developed large edemas .
	manualset3
84304	2	398193	5	NULL	NULL	0	NULL	mutant HNF1B variants P328L329del and A263insGG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat-shock activation of the mutant HNF1B variants P328L329del and A263insGG resulted in malformations of various organs and the affected larvae developed large edemas .
	manualset3
84305	3	398193	5	NULL	NULL	0	NULL	malformations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat-shock activation of the mutant HNF1B variants P328L329del and A263insGG resulted in malformations of various organs and the affected larvae developed large edemas .
	manualset3
84306	4	398193	5	NULL	NULL	0	NULL	various organs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat-shock activation of the mutant HNF1B variants P328L329del and A263insGG resulted in malformations of various organs and the affected larvae developed large edemas .
	manualset3
84307	5	398193	5	NULL	NULL	0	NULL	affected larvae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat-shock activation of the mutant HNF1B variants P328L329del and A263insGG resulted in malformations of various organs and the affected larvae developed large edemas .
	manualset3
84308	6	398193	5	NULL	NULL	0	NULL	edemas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat-shock activation of the mutant HNF1B variants P328L329del and A263insGG resulted in malformations of various organs and the affected larvae developed large edemas .
	manualset3
84309	1	398194	5	NULL	NULL	0	NULL	Heat-stressed 44-59-day-old quails	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat-stressed 44-59-day-old quails elevated their Tb to as much as an average 44.1 degrees C in Ta of about 45 degrees C. The obtained growth model and a gradual development of the body temperature regulation mechanism in king quails followed the known strategy of development , typical for precocial birds .
	manualset3
84310	2	398194	5	NULL	NULL	NULL	NULL	Tb	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Heat-stressed 44-59-day-old quails elevated their Tb to as much as an average 44.1 degrees C in Ta of about 45 degrees C. The obtained growth model and a gradual development of the body temperature regulation mechanism in king quails followed the known strategy of development , typical for precocial birds .
	manualset3
84311	3	398194	5	NULL	NULL	0	NULL	44.1 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat-stressed 44-59-day-old quails elevated their Tb to as much as an average 44.1 degrees C in Ta of about 45 degrees C. The obtained growth model and a gradual development of the body temperature regulation mechanism in king quails followed the known strategy of development , typical for precocial birds .
	manualset3
84312	4	398194	5	NULL	NULL	0	NULL	Ta	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat-stressed 44-59-day-old quails elevated their Tb to as much as an average 44.1 degrees C in Ta of about 45 degrees C. The obtained growth model and a gradual development of the body temperature regulation mechanism in king quails followed the known strategy of development , typical for precocial birds .
	manualset3
84313	5	398194	5	NULL	NULL	0	NULL	45 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat-stressed 44-59-day-old quails elevated their Tb to as much as an average 44.1 degrees C in Ta of about 45 degrees C. The obtained growth model and a gradual development of the body temperature regulation mechanism in king quails followed the known strategy of development , typical for precocial birds .
	manualset3
84314	6	398194	5	NULL	NULL	0	NULL	obtained growth model 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat-stressed 44-59-day-old quails elevated their Tb to as much as an average 44.1 degrees C in Ta of about 45 degrees C. The obtained growth model and a gradual development of the body temperature regulation mechanism in king quails followed the known strategy of development , typical for precocial birds .
	manualset3
84315	7	398194	5	NULL	NULL	0	NULL	gradual development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat-stressed 44-59-day-old quails elevated their Tb to as much as an average 44.1 degrees C in Ta of about 45 degrees C. The obtained growth model and a gradual development of the body temperature regulation mechanism in king quails followed the known strategy of development , typical for precocial birds .
	manualset3
84316	8	398194	5	NULL	NULL	0	NULL	body temperature regulation mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat-stressed 44-59-day-old quails elevated their Tb to as much as an average 44.1 degrees C in Ta of about 45 degrees C. The obtained growth model and a gradual development of the body temperature regulation mechanism in king quails followed the known strategy of development , typical for precocial birds .
	manualset3
84317	9	398194	5	NULL	NULL	0	NULL	king quails	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat-stressed 44-59-day-old quails elevated their Tb to as much as an average 44.1 degrees C in Ta of about 45 degrees C. The obtained growth model and a gradual development of the body temperature regulation mechanism in king quails followed the known strategy of development , typical for precocial birds .
	manualset3
84318	10	398194	5	NULL	NULL	0	NULL	known strategy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat-stressed 44-59-day-old quails elevated their Tb to as much as an average 44.1 degrees C in Ta of about 45 degrees C. The obtained growth model and a gradual development of the body temperature regulation mechanism in king quails followed the known strategy of development , typical for precocial birds .
	manualset3
84319	11	398194	5	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat-stressed 44-59-day-old quails elevated their Tb to as much as an average 44.1 degrees C in Ta of about 45 degrees C. The obtained growth model and a gradual development of the body temperature regulation mechanism in king quails followed the known strategy of development , typical for precocial birds .
	manualset3
84320	12	398194	5	NULL	NULL	0	NULL	precocial birds	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat-stressed 44-59-day-old quails elevated their Tb to as much as an average 44.1 degrees C in Ta of about 45 degrees C. The obtained growth model and a gradual development of the body temperature regulation mechanism in king quails followed the known strategy of development , typical for precocial birds .
	manualset3
84321	1	398195	5	NULL	NULL	0	NULL	Heat protection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat protection was principally reflected in an increased Dq on the 45 degrees C survival curve ; for example , with 100 mM L-alanine , the Dq increased from approximately equal to 20 ( control ) to 30 min at 45 degrees C. Hyperthermia of 1 h at temperatures between 42 degrees C and 45 degrees C indicated that 100 mM alanine had shifted the isotoxic temperature by 0.5 degrees C. Comparable heat protection was also observed with D-alanine and amino acid dimers , such as alanyl-alanine or alanyl-leucine .
	manualset3
84322	2	398195	5	NULL	NULL	0	NULL	increased Dq	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat protection was principally reflected in an increased Dq on the 45 degrees C survival curve ; for example , with 100 mM L-alanine , the Dq increased from approximately equal to 20 ( control ) to 30 min at 45 degrees C. Hyperthermia of 1 h at temperatures between 42 degrees C and 45 degrees C indicated that 100 mM alanine had shifted the isotoxic temperature by 0.5 degrees C. Comparable heat protection was also observed with D-alanine and amino acid dimers , such as alanyl-alanine or alanyl-leucine .
	manualset3
84323	3	398195	5	NULL	NULL	0	NULL	45 degrees C survival curve	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat protection was principally reflected in an increased Dq on the 45 degrees C survival curve ; for example , with 100 mM L-alanine , the Dq increased from approximately equal to 20 ( control ) to 30 min at 45 degrees C. Hyperthermia of 1 h at temperatures between 42 degrees C and 45 degrees C indicated that 100 mM alanine had shifted the isotoxic temperature by 0.5 degrees C. Comparable heat protection was also observed with D-alanine and amino acid dimers , such as alanyl-alanine or alanyl-leucine .
	manualset3
84324	4	398195	5	NULL	NULL	0	NULL	100 mM L-alanine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat protection was principally reflected in an increased Dq on the 45 degrees C survival curve ; for example , with 100 mM L-alanine , the Dq increased from approximately equal to 20 ( control ) to 30 min at 45 degrees C. Hyperthermia of 1 h at temperatures between 42 degrees C and 45 degrees C indicated that 100 mM alanine had shifted the isotoxic temperature by 0.5 degrees C. Comparable heat protection was also observed with D-alanine and amino acid dimers , such as alanyl-alanine or alanyl-leucine .
	manualset3
84325	5	398195	5	NULL	NULL	0	NULL	Dq	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat protection was principally reflected in an increased Dq on the 45 degrees C survival curve ; for example , with 100 mM L-alanine , the Dq increased from approximately equal to 20 ( control ) to 30 min at 45 degrees C. Hyperthermia of 1 h at temperatures between 42 degrees C and 45 degrees C indicated that 100 mM alanine had shifted the isotoxic temperature by 0.5 degrees C. Comparable heat protection was also observed with D-alanine and amino acid dimers , such as alanyl-alanine or alanyl-leucine .
	manualset3
84326	6	398195	5	NULL	NULL	0	NULL	20 ( control ) to 30 min at 45 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat protection was principally reflected in an increased Dq on the 45 degrees C survival curve ; for example , with 100 mM L-alanine , the Dq increased from approximately equal to 20 ( control ) to 30 min at 45 degrees C. Hyperthermia of 1 h at temperatures between 42 degrees C and 45 degrees C indicated that 100 mM alanine had shifted the isotoxic temperature by 0.5 degrees C. Comparable heat protection was also observed with D-alanine and amino acid dimers , such as alanyl-alanine or alanyl-leucine .
	manualset3
84327	7	398195	5	NULL	NULL	0	NULL	Hyperthermia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat protection was principally reflected in an increased Dq on the 45 degrees C survival curve ; for example , with 100 mM L-alanine , the Dq increased from approximately equal to 20 ( control ) to 30 min at 45 degrees C. Hyperthermia of 1 h at temperatures between 42 degrees C and 45 degrees C indicated that 100 mM alanine had shifted the isotoxic temperature by 0.5 degrees C. Comparable heat protection was also observed with D-alanine and amino acid dimers , such as alanyl-alanine or alanyl-leucine .
	manualset3
84328	8	398195	5	NULL	NULL	0	NULL	1 h	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat protection was principally reflected in an increased Dq on the 45 degrees C survival curve ; for example , with 100 mM L-alanine , the Dq increased from approximately equal to 20 ( control ) to 30 min at 45 degrees C. Hyperthermia of 1 h at temperatures between 42 degrees C and 45 degrees C indicated that 100 mM alanine had shifted the isotoxic temperature by 0.5 degrees C. Comparable heat protection was also observed with D-alanine and amino acid dimers , such as alanyl-alanine or alanyl-leucine .
	manualset3
84329	9	398195	5	NULL	NULL	0	NULL	temperatures between 42 degrees C and 45 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat protection was principally reflected in an increased Dq on the 45 degrees C survival curve ; for example , with 100 mM L-alanine , the Dq increased from approximately equal to 20 ( control ) to 30 min at 45 degrees C. Hyperthermia of 1 h at temperatures between 42 degrees C and 45 degrees C indicated that 100 mM alanine had shifted the isotoxic temperature by 0.5 degrees C. Comparable heat protection was also observed with D-alanine and amino acid dimers , such as alanyl-alanine or alanyl-leucine .
	manualset3
84330	10	398195	5	NULL	NULL	0	NULL	100 mM alanine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat protection was principally reflected in an increased Dq on the 45 degrees C survival curve ; for example , with 100 mM L-alanine , the Dq increased from approximately equal to 20 ( control ) to 30 min at 45 degrees C. Hyperthermia of 1 h at temperatures between 42 degrees C and 45 degrees C indicated that 100 mM alanine had shifted the isotoxic temperature by 0.5 degrees C. Comparable heat protection was also observed with D-alanine and amino acid dimers , such as alanyl-alanine or alanyl-leucine .
	manualset3
84331	11	398195	5	NULL	NULL	0	NULL	isotoxic temperature	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat protection was principally reflected in an increased Dq on the 45 degrees C survival curve ; for example , with 100 mM L-alanine , the Dq increased from approximately equal to 20 ( control ) to 30 min at 45 degrees C. Hyperthermia of 1 h at temperatures between 42 degrees C and 45 degrees C indicated that 100 mM alanine had shifted the isotoxic temperature by 0.5 degrees C. Comparable heat protection was also observed with D-alanine and amino acid dimers , such as alanyl-alanine or alanyl-leucine .
	manualset3
84332	12	398195	5	NULL	NULL	0	NULL	0.5 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat protection was principally reflected in an increased Dq on the 45 degrees C survival curve ; for example , with 100 mM L-alanine , the Dq increased from approximately equal to 20 ( control ) to 30 min at 45 degrees C. Hyperthermia of 1 h at temperatures between 42 degrees C and 45 degrees C indicated that 100 mM alanine had shifted the isotoxic temperature by 0.5 degrees C. Comparable heat protection was also observed with D-alanine and amino acid dimers , such as alanyl-alanine or alanyl-leucine .
	manualset3
84333	13	398195	5	NULL	NULL	0	NULL	Comparable heat protection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat protection was principally reflected in an increased Dq on the 45 degrees C survival curve ; for example , with 100 mM L-alanine , the Dq increased from approximately equal to 20 ( control ) to 30 min at 45 degrees C. Hyperthermia of 1 h at temperatures between 42 degrees C and 45 degrees C indicated that 100 mM alanine had shifted the isotoxic temperature by 0.5 degrees C. Comparable heat protection was also observed with D-alanine and amino acid dimers , such as alanyl-alanine or alanyl-leucine .
	manualset3
84334	14	398195	5	NULL	NULL	0	NULL	D-alanine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat protection was principally reflected in an increased Dq on the 45 degrees C survival curve ; for example , with 100 mM L-alanine , the Dq increased from approximately equal to 20 ( control ) to 30 min at 45 degrees C. Hyperthermia of 1 h at temperatures between 42 degrees C and 45 degrees C indicated that 100 mM alanine had shifted the isotoxic temperature by 0.5 degrees C. Comparable heat protection was also observed with D-alanine and amino acid dimers , such as alanyl-alanine or alanyl-leucine .
	manualset3
84335	15	398195	5	NULL	NULL	0	NULL	amino acid dimers , such as alanyl-alanine or alanyl-leucine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat protection was principally reflected in an increased Dq on the 45 degrees C survival curve ; for example , with 100 mM L-alanine , the Dq increased from approximately equal to 20 ( control ) to 30 min at 45 degrees C. Hyperthermia of 1 h at temperatures between 42 degrees C and 45 degrees C indicated that 100 mM alanine had shifted the isotoxic temperature by 0.5 degrees C. Comparable heat protection was also observed with D-alanine and amino acid dimers , such as alanyl-alanine or alanyl-leucine .
	manualset3
84336	1	398196	5	NULL	NULL	0	NULL	Heat shock	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat shock to embryonal carcinoma cells PCC4 at 45 degrees C for 30 min resulted in the differentiation of cells although heat shock response was induced on exposure to 42 degrees C for 60 min .
	manualset3
84337	2	398196	5	NULL	NULL	0	NULL	embryonal carcinoma cells PCC4 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat shock to embryonal carcinoma cells PCC4 at 45 degrees C for 30 min resulted in the differentiation of cells although heat shock response was induced on exposure to 42 degrees C for 60 min .
	manualset3
84338	3	398196	5	NULL	NULL	0	NULL	45 degrees C 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat shock to embryonal carcinoma cells PCC4 at 45 degrees C for 30 min resulted in the differentiation of cells although heat shock response was induced on exposure to 42 degrees C for 60 min .
	manualset3
84339	4	398196	5	NULL	NULL	0	NULL	30 min	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat shock to embryonal carcinoma cells PCC4 at 45 degrees C for 30 min resulted in the differentiation of cells although heat shock response was induced on exposure to 42 degrees C for 60 min .
	manualset3
84340	5	398196	5	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat shock to embryonal carcinoma cells PCC4 at 45 degrees C for 30 min resulted in the differentiation of cells although heat shock response was induced on exposure to 42 degrees C for 60 min .
	manualset3
84341	6	398196	5	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat shock to embryonal carcinoma cells PCC4 at 45 degrees C for 30 min resulted in the differentiation of cells although heat shock response was induced on exposure to 42 degrees C for 60 min .
	manualset3
84342	7	398196	5	NULL	NULL	0	NULL	heat shock response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat shock to embryonal carcinoma cells PCC4 at 45 degrees C for 30 min resulted in the differentiation of cells although heat shock response was induced on exposure to 42 degrees C for 60 min .
	manualset3
84343	8	398196	5	NULL	NULL	0	NULL	42 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat shock to embryonal carcinoma cells PCC4 at 45 degrees C for 30 min resulted in the differentiation of cells although heat shock response was induced on exposure to 42 degrees C for 60 min .
	manualset3
84344	9	398196	5	NULL	NULL	0	NULL	60 min	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat shock to embryonal carcinoma cells PCC4 at 45 degrees C for 30 min resulted in the differentiation of cells although heat shock response was induced on exposure to 42 degrees C for 60 min .
	manualset3
84345	1	398197	5	NULL	NULL	0	NULL	lidocaine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Heating lidocaine appears to prevent painful injection .
	manualset3
84346	2	398197	5	NULL	NULL	0	NULL	painful injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Heating lidocaine appears to prevent painful injection .
	manualset3
84347	1	398198	5	NULL	NULL	0	NULL	ethylene oxide sterilization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heating during ethylene oxide sterilization also resulted in reduced viscosity and breakdown .
	manualset3
84348	2	398198	5	NULL	NULL	NULL	NULL	reduced viscosity and breakdown	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Heating during ethylene oxide sterilization also resulted in reduced viscosity and breakdown .
	manualset3
84349	2	398199	5	NULL	NULL	NULL	NULL	lipoid-reagin	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Heating the lipoid-reagin precipitate to 100 degrees for 1 minute destroys the sensitizing film of reagin globulin ; the avidity for complement disappears simultaneously .
	manualset3
84350	3	398199	5	NULL	NULL	NULL	NULL	100 degrees	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Heating the lipoid-reagin precipitate to 100 degrees for 1 minute destroys the sensitizing film of reagin globulin ; the avidity for complement disappears simultaneously .
	manualset3
84351	4	398199	5	NULL	NULL	NULL	NULL	1 minute	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Heating the lipoid-reagin precipitate to 100 degrees for 1 minute destroys the sensitizing film of reagin globulin ; the avidity for complement disappears simultaneously .
	manualset3
84353	5	398199	5	NULL	NULL	0	NULL	reagin globulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Heating the lipoid-reagin precipitate to 100 degrees for 1 minute destroys the sensitizing film of reagin globulin ; the avidity for complement disappears simultaneously .
	manualset3
84354	6	398199	5	NULL	NULL	0	NULL	avidity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heating the lipoid-reagin precipitate to 100 degrees for 1 minute destroys the sensitizing film of reagin globulin ; the avidity for complement disappears simultaneously .
	manualset3
84355	7	398199	5	NULL	NULL	0	NULL	complement	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Heating the lipoid-reagin precipitate to 100 degrees for 1 minute destroys the sensitizing film of reagin globulin ; the avidity for complement disappears simultaneously .
	manualset3
84503	1	398199	5	NULL	NULL	0	NULL	Heating	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Heating the lipoid-reagin precipitate to 100 degrees for 1 minute destroys the sensitizing film of reagin globulin ; the avidity for complement disappears simultaneously .
	manualset3
84356	1	398200	5	NULL	NULL	0	NULL	Heavy meromyosin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Heavy meromyosin induces sliding movements between antiparallel actin filaments .
	manualset3
84357	2	398200	5	NULL	NULL	0	NULL	sliding movements	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heavy meromyosin induces sliding movements between antiparallel actin filaments .
	manualset3
84358	3	398200	5	NULL	NULL	NULL	NULL	antiparallel actin filaments	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Heavy meromyosin induces sliding movements between antiparallel actin filaments .
	manualset3
84359	1	398201	5	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on uric acid metabolism in various skin diseases ( supplemental report ) .
	manualset3
84360	2	398201	5	NULL	NULL	0	NULL	uric acid metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on uric acid metabolism in various skin diseases ( supplemental report ) .
	manualset3
84361	3	398201	5	NULL	NULL	0	NULL	skin diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on uric acid metabolism in various skin diseases ( supplemental report ) .
	manualset3
84362	4	398201	5	NULL	NULL	0	NULL	supplemental report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on uric acid metabolism in various skin diseases ( supplemental report ) .
	manualset3
84363	1	398202	5	NULL	NULL	0	NULL	Heifers	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Heifers fed accelerated diets had a higher average daily gain ( 933 vs. 778 g/d ) and calved earlier ( 21.7 vs. 24.6 mo ) than did heifers fed control diets .
	manualset3
84364	2	398202	5	NULL	NULL	0	NULL	accelerated diets	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Heifers fed accelerated diets had a higher average daily gain ( 933 vs. 778 g/d ) and calved earlier ( 21.7 vs. 24.6 mo ) than did heifers fed control diets .
	manualset3
84365	3	398202	5	NULL	NULL	0	NULL	 higher average daily gain ( 933 vs. 778 g/d )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Heifers fed accelerated diets had a higher average daily gain ( 933 vs. 778 g/d ) and calved earlier ( 21.7 vs. 24.6 mo ) than did heifers fed control diets .
	manualset3
84366	4	398202	5	NULL	NULL	0	NULL	calved earlier ( 21.7 vs. 24.6 mo )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Heifers fed accelerated diets had a higher average daily gain ( 933 vs. 778 g/d ) and calved earlier ( 21.7 vs. 24.6 mo ) than did heifers fed control diets .
	manualset3
84367	5	398202	5	NULL	NULL	0	NULL	heifers	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Heifers fed accelerated diets had a higher average daily gain ( 933 vs. 778 g/d ) and calved earlier ( 21.7 vs. 24.6 mo ) than did heifers fed control diets .
	manualset3
84368	6	398202	5	NULL	NULL	0	NULL	control diets	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Heifers fed accelerated diets had a higher average daily gain ( 933 vs. 778 g/d ) and calved earlier ( 21.7 vs. 24.6 mo ) than did heifers fed control diets .
	manualset3
84369	1	398203	5	NULL	NULL	0	NULL	Heifers	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Heifers were injected in the area of the supramammary lymph nodes with vaccine or placebo twice before calving and observed and sampled throughout their first lactation .
	manualset3
84370	2	398203	5	NULL	NULL	0	NULL	area of the supramammary lymph nodes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Heifers were injected in the area of the supramammary lymph nodes with vaccine or placebo twice before calving and observed and sampled throughout their first lactation .
	manualset3
84371	3	398203	5	NULL	NULL	0	NULL	vaccine	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Heifers were injected in the area of the supramammary lymph nodes with vaccine or placebo twice before calving and observed and sampled throughout their first lactation .
	manualset3
84372	4	398203	5	NULL	NULL	0	NULL	placebo	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Heifers were injected in the area of the supramammary lymph nodes with vaccine or placebo twice before calving and observed and sampled throughout their first lactation .
	manualset3
84373	5	398203	5	NULL	NULL	0	NULL	first lactation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heifers were injected in the area of the supramammary lymph nodes with vaccine or placebo twice before calving and observed and sampled throughout their first lactation .
	manualset3
84374	1	398204	5	NULL	NULL	0	NULL	Heifers	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Heifers were inseminated at 6 h and 16 h after onset of estrus .
	manualset3
84375	2	398204	5	NULL	NULL	0	NULL	6 h and 16 h	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Heifers were inseminated at 6 h and 16 h after onset of estrus .
	manualset3
84376	3	398204	5	NULL	NULL	0	NULL	estrus	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heifers were inseminated at 6 h and 16 h after onset of estrus .
	manualset3
84377	1	398205	5	NULL	NULL	0	NULL	Height gain	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Height gain can be successfully achieved in these patients with growth hormone treatment .
	manualset3
84378	2	398205	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Height gain can be successfully achieved in these patients with growth hormone treatment .
	manualset3
84379	3	398205	5	NULL	NULL	0	NULL	growth hormone treatment	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Height gain can be successfully achieved in these patients with growth hormone treatment .
	manualset3
84380	1	398206	5	NULL	NULL	0	NULL	Helicity propensity and interaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Helicity propensity and interaction of synthetic peptides from heptad-repeat domains of herpes simplex virus 1 glycoprotein H : a circular dichroism study .
	manualset3
84381	2	398206	5	NULL	NULL	0	NULL	synthetic peptides	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Helicity propensity and interaction of synthetic peptides from heptad-repeat domains of herpes simplex virus 1 glycoprotein H : a circular dichroism study .
	manualset3
84382	3	398206	5	NULL	NULL	0	NULL	heptad-repeat domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Helicity propensity and interaction of synthetic peptides from heptad-repeat domains of herpes simplex virus 1 glycoprotein H : a circular dichroism study .
	manualset3
84383	4	398206	5	NULL	NULL	0	NULL	herpes simplex virus 1 glycoprotein H	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Helicity propensity and interaction of synthetic peptides from heptad-repeat domains of herpes simplex virus 1 glycoprotein H : a circular dichroism study .
	manualset3
84384	5	398206	5	NULL	NULL	0	NULL	circular dichroism study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Helicity propensity and interaction of synthetic peptides from heptad-repeat domains of herpes simplex virus 1 glycoprotein H : a circular dichroism study .
	manualset3
84385	1	398207	5	NULL	NULL	0	NULL	Helicobacter pylori	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Helicobacter pylori induces the release of alpha-defensin by human granulocytes .
	manualset3
84386	2	398207	5	NULL	NULL	0	NULL	alpha-defensin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Helicobacter pylori induces the release of alpha-defensin by human granulocytes .
	manualset3
84387	3	398207	5	NULL	NULL	0	NULL	human granulocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Helicobacter pylori induces the release of alpha-defensin by human granulocytes .
	manualset3
84388	1	398208	5	NULL	NULL	0	NULL	Helicobacter pylori infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Helicobacter pylori infection : a risk factor for ischaemic cerebrovascular disease and carotid atheroma .
	manualset3
84389	2	398208	5	NULL	NULL	0	NULL	ischaemic cerebrovascular disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Helicobacter pylori infection : a risk factor for ischaemic cerebrovascular disease and carotid atheroma .
	manualset3
84390	3	398208	5	NULL	NULL	0	NULL	carotid atheroma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Helicobacter pylori infection : a risk factor for ischaemic cerebrovascular disease and carotid atheroma .
	manualset3
84391	1	398209	5	NULL	NULL	0	NULL	Helicobacter pylori	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Helicobacter pylori is the definitive carcinogen for stomach cancer and is known to induce proinflammatory cytokines , such as tumor necrosis factor-alpha ( TNF-alpha ) and interleukin-1 ( IL-1 ) in the stomach .
	manualset3
84392	2	398209	5	NULL	NULL	0	NULL	definitive carcinogen	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Helicobacter pylori is the definitive carcinogen for stomach cancer and is known to induce proinflammatory cytokines , such as tumor necrosis factor-alpha ( TNF-alpha ) and interleukin-1 ( IL-1 ) in the stomach .
	manualset3
84393	3	398209	5	NULL	NULL	0	NULL	stomach cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Helicobacter pylori is the definitive carcinogen for stomach cancer and is known to induce proinflammatory cytokines , such as tumor necrosis factor-alpha ( TNF-alpha ) and interleukin-1 ( IL-1 ) in the stomach .
	manualset3
84394	4	398209	5	NULL	NULL	0	NULL	proinflammatory cytokines	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Helicobacter pylori is the definitive carcinogen for stomach cancer and is known to induce proinflammatory cytokines , such as tumor necrosis factor-alpha ( TNF-alpha ) and interleukin-1 ( IL-1 ) in the stomach .
	manualset3
84395	5	398209	5	NULL	NULL	0	NULL	tumor necrosis factor-alpha ( TNF-alpha )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Helicobacter pylori is the definitive carcinogen for stomach cancer and is known to induce proinflammatory cytokines , such as tumor necrosis factor-alpha ( TNF-alpha ) and interleukin-1 ( IL-1 ) in the stomach .
	manualset3
84396	6	398209	5	NULL	NULL	0	NULL	interleukin-1 ( IL-1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Helicobacter pylori is the definitive carcinogen for stomach cancer and is known to induce proinflammatory cytokines , such as tumor necrosis factor-alpha ( TNF-alpha ) and interleukin-1 ( IL-1 ) in the stomach .
	manualset3
84397	7	398209	5	NULL	NULL	0	NULL	stomach	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Helicobacter pylori is the definitive carcinogen for stomach cancer and is known to induce proinflammatory cytokines , such as tumor necrosis factor-alpha ( TNF-alpha ) and interleukin-1 ( IL-1 ) in the stomach .
	manualset3
84398	1	398210	5	NULL	NULL	0	NULL	Study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Study of Morita therapy -- including an experience in participating a joint study program for young psychiatrists from Japan and Korea ) .
	manualset3
84399	2	398210	5	NULL	NULL	0	NULL	Morita therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Study of Morita therapy -- including an experience in participating a joint study program for young psychiatrists from Japan and Korea ) .
	manualset3
84400	3	398210	5	NULL	NULL	0	NULL	experience	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Study of Morita therapy -- including an experience in participating a joint study program for young psychiatrists from Japan and Korea ) .
	manualset3
84401	4	398210	5	NULL	NULL	0	NULL	joint study program	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Study of Morita therapy -- including an experience in participating a joint study program for young psychiatrists from Japan and Korea ) .
	manualset3
84402	5	398210	5	NULL	NULL	0	NULL	young psychiatrists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Study of Morita therapy -- including an experience in participating a joint study program for young psychiatrists from Japan and Korea ) .
	manualset3
84403	6	398210	5	NULL	NULL	0	NULL	Japan and Korea	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Study of Morita therapy -- including an experience in participating a joint study program for young psychiatrists from Japan and Korea ) .
	manualset3
84404	1	398211	5	NULL	NULL	0	NULL	Hema-Strip HIV-1 / 2	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hema-Strip HIV-1 / 2 is a one-step rapid test for the detection of anti-HIV-1 / 2 antibodies in whole blood .
	manualset3
84405	2	398211	5	NULL	NULL	0	NULL	one-step rapid test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hema-Strip HIV-1 / 2 is a one-step rapid test for the detection of anti-HIV-1 / 2 antibodies in whole blood .
	manualset3
84406	3	398211	5	NULL	NULL	0	NULL	detection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hema-Strip HIV-1 / 2 is a one-step rapid test for the detection of anti-HIV-1 / 2 antibodies in whole blood .
	manualset3
84407	4	398211	5	NULL	NULL	0	NULL	anti-HIV-1 / 2 antibodies	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hema-Strip HIV-1 / 2 is a one-step rapid test for the detection of anti-HIV-1 / 2 antibodies in whole blood .
	manualset3
84408	5	398211	5	NULL	NULL	0	NULL	whole blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Hema-Strip HIV-1 / 2 is a one-step rapid test for the detection of anti-HIV-1 / 2 antibodies in whole blood .
	manualset3
84409	1	398212	5	NULL	NULL	0	NULL	Hemangiomatosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemangiomatosis of the liver is growing in the last decades , because of the abdominal imaging progresses : brain CT scan , MRI .
	manualset3
84410	2	398212	5	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemangiomatosis of the liver is growing in the last decades , because of the abdominal imaging progresses : brain CT scan , MRI .
	manualset3
84411	3	398212	5	NULL	NULL	0	NULL	last decades	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemangiomatosis of the liver is growing in the last decades , because of the abdominal imaging progresses : brain CT scan , MRI .
	manualset3
84412	4	398212	5	NULL	NULL	NULL	NULL	abdominal imaging progresses	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hemangiomatosis of the liver is growing in the last decades , because of the abdominal imaging progresses : brain CT scan , MRI .
	manualset3
84413	5	398212	5	NULL	NULL	NULL	NULL	brain CT scan	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hemangiomatosis of the liver is growing in the last decades , because of the abdominal imaging progresses : brain CT scan , MRI .
	manualset3
84414	6	398212	5	NULL	NULL	0	NULL	MRI	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemangiomatosis of the liver is growing in the last decades , because of the abdominal imaging progresses : brain CT scan , MRI .
	manualset3
84415	1	398213	5	NULL	NULL	0	NULL	Hemangiopericytoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemangiopericytoma of the orbit treated with conservative surgery and radiotherapy .
	manualset3
84416	2	398213	5	NULL	NULL	0	NULL	orbit	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemangiopericytoma of the orbit treated with conservative surgery and radiotherapy .
	manualset3
84417	3	398213	5	NULL	NULL	NULL	NULL	conservative surgery and radiotherapy 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hemangiopericytoma of the orbit treated with conservative surgery and radiotherapy .
	manualset3
84418	1	398214	5	NULL	NULL	0	NULL	Hemato-vascular origins	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemato-vascular origins of endothelial progenitor cells ?
	manualset3
84419	2	398214	5	NULL	NULL	0	NULL	endothelial progenitor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemato-vascular origins of endothelial progenitor cells ?
	manualset3
84420	1	398215	5	NULL	NULL	0	NULL	Hematological malignancie	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hematological malignancies in the island of Sardinia , 1974-1993 : age and sex distributions and temporal changes in incidence .
	manualset3
84421	2	398215	5	NULL	NULL	0	NULL	island of Sardinia	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Hematological malignancies in the island of Sardinia , 1974-1993 : age and sex distributions and temporal changes in incidence .
	manualset3
84422	3	398215	5	NULL	NULL	0	NULL	1974-1993	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Hematological malignancies in the island of Sardinia , 1974-1993 : age and sex distributions and temporal changes in incidence .
	manualset3
84423	4	398215	5	NULL	NULL	0	NULL	age and sex distributions	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Hematological malignancies in the island of Sardinia , 1974-1993 : age and sex distributions and temporal changes in incidence .
	manualset3
84424	5	398215	5	NULL	NULL	0	NULL	temporal changes in incidence	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Hematological malignancies in the island of Sardinia , 1974-1993 : age and sex distributions and temporal changes in incidence .
	manualset3
84425	1	398216	5	NULL	NULL	0	NULL	Hematopoietic SCT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hematopoietic SCT became an established therapy for such disorders .
	manualset3
84426	2	398216	5	NULL	NULL	0	NULL	established therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hematopoietic SCT became an established therapy for such disorders .
	manualset3
84427	3	398216	5	NULL	NULL	0	NULL	disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hematopoietic SCT became an established therapy for such disorders .
	manualset3
84428	1	398217	5	NULL	NULL	0	NULL	Hematopoietic stem/progenitor cells ( HSPCs )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Hematopoietic stem/progenitor cells ( HSPCs ) in placental/umbilical cord blood ( CB ) , which is neonatal peripheral blood , have increasingly been used for hematopoietic stem cell transplantations .
	manualset3
84429	2	398217	5	NULL	NULL	0	NULL	placental/umbilical cord blood ( CB )	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Hematopoietic stem/progenitor cells ( HSPCs ) in placental/umbilical cord blood ( CB ) , which is neonatal peripheral blood , have increasingly been used for hematopoietic stem cell transplantations .
	manualset3
84430	3	398217	5	NULL	NULL	0	NULL	neonatal peripheral blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Hematopoietic stem/progenitor cells ( HSPCs ) in placental/umbilical cord blood ( CB ) , which is neonatal peripheral blood , have increasingly been used for hematopoietic stem cell transplantations .
	manualset3
84431	4	398217	5	NULL	NULL	0	NULL	hematopoietic stem cell transplantations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hematopoietic stem/progenitor cells ( HSPCs ) in placental/umbilical cord blood ( CB ) , which is neonatal peripheral blood , have increasingly been used for hematopoietic stem cell transplantations .
	manualset3
84432	1	398218	5	NULL	NULL	0	NULL	Hematuria	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hematuria was relatively frequent ( 33 % in the Fraxiparine group and 28 % in the Calciparine group ) , however these rates were related to prostatic and urinary incontinence surgery .
	manualset3
84433	2	398218	5	NULL	NULL	0	NULL	33 % in the Fraxiparine group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hematuria was relatively frequent ( 33 % in the Fraxiparine group and 28 % in the Calciparine group ) , however these rates were related to prostatic and urinary incontinence surgery .
	manualset3
84434	3	398218	5	NULL	NULL	0	NULL	28 % in the Calciparine group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hematuria was relatively frequent ( 33 % in the Fraxiparine group and 28 % in the Calciparine group ) , however these rates were related to prostatic and urinary incontinence surgery .
	manualset3
84435	4	398218	5	NULL	NULL	0	NULL	prostatic and urinary incontinence surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hematuria was relatively frequent ( 33 % in the Fraxiparine group and 28 % in the Calciparine group ) , however these rates were related to prostatic and urinary incontinence surgery .
	manualset3
84436	1	398219	5	NULL	NULL	0	NULL	Heme oxygenase-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Heme oxygenase-1 stabilizes the blood-spinal cord barrier and limits oxidative stress and white matter damage in the acutely injured murine spinal cord .
	manualset3
84437	2	398219	5	NULL	NULL	0	NULL	blood-spinal cord barrier	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Heme oxygenase-1 stabilizes the blood-spinal cord barrier and limits oxidative stress and white matter damage in the acutely injured murine spinal cord .
	manualset3
84438	3	398219	5	NULL	NULL	0	NULL	oxidative stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Heme oxygenase-1 stabilizes the blood-spinal cord barrier and limits oxidative stress and white matter damage in the acutely injured murine spinal cord .
	manualset3
84439	4	398219	5	NULL	NULL	0	NULL	white matter damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Heme oxygenase-1 stabilizes the blood-spinal cord barrier and limits oxidative stress and white matter damage in the acutely injured murine spinal cord .
	manualset3
84440	5	398219	5	NULL	NULL	0	NULL	acutely injured murine spinal cord	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Heme oxygenase-1 stabilizes the blood-spinal cord barrier and limits oxidative stress and white matter damage in the acutely injured murine spinal cord .
	manualset3
84441	1	398220	5	NULL	NULL	0	NULL	Hemodialysis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemodialysis elicited marked reduction in early diastolic lateral mitral annular and midlateral myocardial velocities ( 6.9 + / - 3.2 to 6.3 + / - 2.9 cm/s , P & lt ; 0.04 and 6.7 + / - 0.3 to 5.5 + / - 2 cm/s , P & lt ; 0.001 , respectively ) .
	manualset3
84442	2	398220	5	NULL	NULL	0	NULL	early diastolic lateral mitral annular and midlateral myocardial velocities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemodialysis elicited marked reduction in early diastolic lateral mitral annular and midlateral myocardial velocities ( 6.9 + / - 3.2 to 6.3 + / - 2.9 cm/s , P & lt ; 0.04 and 6.7 + / - 0.3 to 5.5 + / - 2 cm/s , P & lt ; 0.001 , respectively ) .
	manualset3
84443	3	398220	5	NULL	NULL	0	NULL	6.9 + / - 3.2 to 6.3 + / - 2.9 cm/s , P & lt ; 0.04 and 6.7 + / - 0.3 to 5.5 + / - 2 cm/s , P & lt ; 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemodialysis elicited marked reduction in early diastolic lateral mitral annular and midlateral myocardial velocities ( 6.9 + / - 3.2 to 6.3 + / - 2.9 cm/s , P & lt ; 0.04 and 6.7 + / - 0.3 to 5.5 + / - 2 cm/s , P & lt ; 0.001 , respectively ) .
	manualset3
84444	1	398221	5	NULL	NULL	0	NULL	Hemodynamic data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemodynamic data indicated that LV function in group A was enhanced during the development of the hypertrophy .
	manualset3
84445	2	398221	5	NULL	NULL	0	NULL	LV function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemodynamic data indicated that LV function in group A was enhanced during the development of the hypertrophy .
	manualset3
84446	3	398221	5	NULL	NULL	0	NULL	group A	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemodynamic data indicated that LV function in group A was enhanced during the development of the hypertrophy .
	manualset3
84447	4	398221	5	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemodynamic data indicated that LV function in group A was enhanced during the development of the hypertrophy .
	manualset3
84448	5	398221	5	NULL	NULL	0	NULL	hypertrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemodynamic data indicated that LV function in group A was enhanced during the development of the hypertrophy .
	manualset3
84449	1	398222	5	NULL	NULL	0	NULL	Hemodynamic improvement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemodynamic improvement was sustained in both dogs at the time of recatheterization 3 months later .
	manualset3
84450	2	398222	5	NULL	NULL	0	NULL	both dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemodynamic improvement was sustained in both dogs at the time of recatheterization 3 months later .
	manualset3
84451	3	398222	5	NULL	NULL	0	NULL	recatheterization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemodynamic improvement was sustained in both dogs at the time of recatheterization 3 months later .
	manualset3
84452	4	398222	5	NULL	NULL	0	NULL	3 months later	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemodynamic improvement was sustained in both dogs at the time of recatheterization 3 months later .
	manualset3
84453	1	398223	5	NULL	NULL	0	NULL	Hemofiltration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemofiltration in human sepsis : evidence for elimination of immunomodulatory substances .
	manualset3
84454	2	398223	5	NULL	NULL	0	NULL	human sepsis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemofiltration in human sepsis : evidence for elimination of immunomodulatory substances .
	manualset3
84455	3	398223	5	NULL	NULL	NULL	NULL	elimination	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hemofiltration in human sepsis : evidence for elimination of immunomodulatory substances .
	manualset3
84456	4	398223	5	NULL	NULL	0	NULL	immunomodulatory substances	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemofiltration in human sepsis : evidence for elimination of immunomodulatory substances .
	manualset3
84457	1	398224	5	NULL	NULL	0	NULL	Hemoglobin G Saskatoon	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemoglobin G Saskatoon : beta-22Glu -- Ala .
	manualset3
84458	2	398224	5	NULL	NULL	0	NULL	beta-22Glu -- Ala	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemoglobin G Saskatoon : beta-22Glu -- Ala .
	manualset3
84459	1	398225	5	NULL	NULL	0	NULL	Hemoglobin ( Hb ) variants	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemoglobin ( Hb ) variants caused by an elongation of the beta-globin chain are rare .
	manualset3
84460	2	398225	5	NULL	NULL	0	NULL	elongation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemoglobin ( Hb ) variants caused by an elongation of the beta-globin chain are rare .
	manualset3
84461	3	398225	5	NULL	NULL	0	NULL	beta-globin chain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemoglobin ( Hb ) variants caused by an elongation of the beta-globin chain are rare .
	manualset3
84462	1	398226	5	NULL	NULL	0	NULL	Hemoglobin Rainier ( beta ( 145 ) tyrosine -- ) histidine )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemoglobin Rainier ( beta ( 145 ) tyrosine -- ) histidine ) is an abnormal hemoglobin associated with increased oxygen affinity , decreased heme-heme interaction , presence of a Bohr effect , and erythrocytosis , but without obvious clinical sequelae .
	manualset3
84463	2	398226	5	NULL	NULL	0	NULL	abnormal hemoglobin associated with increased oxygen affinity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemoglobin Rainier ( beta ( 145 ) tyrosine -- ) histidine ) is an abnormal hemoglobin associated with increased oxygen affinity , decreased heme-heme interaction , presence of a Bohr effect , and erythrocytosis , but without obvious clinical sequelae .
	manualset3
84464	3	398226	5	NULL	NULL	0	NULL	heme-heme interaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemoglobin Rainier ( beta ( 145 ) tyrosine -- ) histidine ) is an abnormal hemoglobin associated with increased oxygen affinity , decreased heme-heme interaction , presence of a Bohr effect , and erythrocytosis , but without obvious clinical sequelae .
	manualset3
84465	4	398226	5	NULL	NULL	0	NULL	Bohr effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemoglobin Rainier ( beta ( 145 ) tyrosine -- ) histidine ) is an abnormal hemoglobin associated with increased oxygen affinity , decreased heme-heme interaction , presence of a Bohr effect , and erythrocytosis , but without obvious clinical sequelae .
	manualset3
84466	5	398226	5	NULL	NULL	0	NULL	erythrocytosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemoglobin Rainier ( beta ( 145 ) tyrosine -- ) histidine ) is an abnormal hemoglobin associated with increased oxygen affinity , decreased heme-heme interaction , presence of a Bohr effect , and erythrocytosis , but without obvious clinical sequelae .
	manualset3
84467	6	398226	5	NULL	NULL	NULL	NULL	obvious clinical sequelae	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hemoglobin Rainier ( beta ( 145 ) tyrosine -- ) histidine ) is an abnormal hemoglobin associated with increased oxygen affinity , decreased heme-heme interaction , presence of a Bohr effect , and erythrocytosis , but without obvious clinical sequelae .
	manualset3
84468	1	398227	5	NULL	NULL	0	NULL	Hemojuvelin ( Hjv )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemojuvelin ( Hjv ) , a member of the repulsive-guidance molecule ( RGM ) family , upregulates transcription of the iron regulatory hormone hepcidin by activating the bone morphogenetic protein ( BMP ) signaling pathway in mammalian cells .
	manualset3
84469	2	398227	5	NULL	NULL	0	NULL	memeber of repulsive-guidance molecule ( RGM ) family	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemojuvelin ( Hjv ) , a member of the repulsive-guidance molecule ( RGM ) family , upregulates transcription of the iron regulatory hormone hepcidin by activating the bone morphogenetic protein ( BMP ) signaling pathway in mammalian cells .
	manualset3
84470	3	398227	5	NULL	NULL	0	NULL	transcription	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemojuvelin ( Hjv ) , a member of the repulsive-guidance molecule ( RGM ) family , upregulates transcription of the iron regulatory hormone hepcidin by activating the bone morphogenetic protein ( BMP ) signaling pathway in mammalian cells .
	manualset3
84471	4	398227	5	NULL	NULL	0	NULL	iron regulatory hormone hepcidin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemojuvelin ( Hjv ) , a member of the repulsive-guidance molecule ( RGM ) family , upregulates transcription of the iron regulatory hormone hepcidin by activating the bone morphogenetic protein ( BMP ) signaling pathway in mammalian cells .
	manualset3
84472	5	398227	5	NULL	NULL	0	NULL	bone morphogenetic protein ( BMP ) signaling pathway	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemojuvelin ( Hjv ) , a member of the repulsive-guidance molecule ( RGM ) family , upregulates transcription of the iron regulatory hormone hepcidin by activating the bone morphogenetic protein ( BMP ) signaling pathway in mammalian cells .
	manualset3
84473	6	398227	5	NULL	NULL	0	NULL	mammalian cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemojuvelin ( Hjv ) , a member of the repulsive-guidance molecule ( RGM ) family , upregulates transcription of the iron regulatory hormone hepcidin by activating the bone morphogenetic protein ( BMP ) signaling pathway in mammalian cells .
	manualset3
84474	1	398228	5	NULL	NULL	0	NULL	Hemolymph oxygen content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemolymph oxygen content fell dramatically at 9 degrees C to values between 2 % and 12 % of ambient water O ( 2 ) content and had a maximum Po ( 2 ) of around 20 mmHg .
	manualset3
84475	2	398228	5	NULL	NULL	0	NULL	9 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemolymph oxygen content fell dramatically at 9 degrees C to values between 2 % and 12 % of ambient water O ( 2 ) content and had a maximum Po ( 2 ) of around 20 mmHg .
	manualset3
84476	3	398228	5	NULL	NULL	0	NULL	values between 2 % and 12 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemolymph oxygen content fell dramatically at 9 degrees C to values between 2 % and 12 % of ambient water O ( 2 ) content and had a maximum Po ( 2 ) of around 20 mmHg .
	manualset3
84477	4	398228	5	NULL	NULL	0	NULL	ambient water O ( 2 ) content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemolymph oxygen content fell dramatically at 9 degrees C to values between 2 % and 12 % of ambient water O ( 2 ) content and had a maximum Po ( 2 ) of around 20 mmHg .
	manualset3
84478	5	398228	5	NULL	NULL	0	NULL	maximum Po ( 2 )	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemolymph oxygen content fell dramatically at 9 degrees C to values between 2 % and 12 % of ambient water O ( 2 ) content and had a maximum Po ( 2 ) of around 20 mmHg .
	manualset3
84479	6	398228	5	NULL	NULL	0	NULL	20 mmHg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemolymph oxygen content fell dramatically at 9 degrees C to values between 2 % and 12 % of ambient water O ( 2 ) content and had a maximum Po ( 2 ) of around 20 mmHg .
	manualset3
84480	1	398229	5	NULL	NULL	0	NULL	Hemolysis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemolysis , lipemia and icterus in specimens for arterial blood gas analysis .
	manualset3
84481	2	398229	5	NULL	NULL	0	NULL	lipemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemolysis , lipemia and icterus in specimens for arterial blood gas analysis .
	manualset3
84482	3	398229	5	NULL	NULL	0	NULL	icterus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemolysis , lipemia and icterus in specimens for arterial blood gas analysis .
	manualset3
84483	4	398229	5	NULL	NULL	NULL	NULL	specimens	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hemolysis , lipemia and icterus in specimens for arterial blood gas analysis .
	manualset3
84484	5	398229	5	NULL	NULL	0	NULL	arterial blood gas analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemolysis , lipemia and icterus in specimens for arterial blood gas analysis .
	manualset3
84485	1	398230	5	NULL	NULL	0	NULL	Hemolysis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemolysis occurring after exposure to oxygen under high pressure .
	manualset3
84486	2	398230	5	NULL	NULL	0	NULL	exposure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemolysis occurring after exposure to oxygen under high pressure .
	manualset3
84487	3	398230	5	NULL	NULL	0	NULL	oxygen	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemolysis occurring after exposure to oxygen under high pressure .
	manualset3
84488	4	398230	5	NULL	NULL	0	NULL	high pressure	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemolysis occurring after exposure to oxygen under high pressure .
	manualset3
84774	1	398231	5	NULL	NULL	0	NULL	Hemolytic activities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemolytic activities in the central cornea were compared with hemolytic activities in the peripheral cornea for each of the following complement components : C1 , C4 , C2 , C3 , C5 , C6 , and C7 .
	manualset3
84775	2	398231	5	NULL	NULL	0	NULL	central cornea	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemolytic activities in the central cornea were compared with hemolytic activities in the peripheral cornea for each of the following complement components : C1 , C4 , C2 , C3 , C5 , C6 , and C7 .
	manualset3
84776	3	398231	5	NULL	NULL	0	NULL	hemolytic activities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemolytic activities in the central cornea were compared with hemolytic activities in the peripheral cornea for each of the following complement components : C1 , C4 , C2 , C3 , C5 , C6 , and C7 .
	manualset3
84777	4	398231	5	NULL	NULL	0	NULL	peripheral cornea	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemolytic activities in the central cornea were compared with hemolytic activities in the peripheral cornea for each of the following complement components : C1 , C4 , C2 , C3 , C5 , C6 , and C7 .
	manualset3
84778	5	398231	5	NULL	NULL	NULL	NULL	complement components : C1 , C4 , C2 , C3 , C5 , C6 , and C7	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hemolytic activities in the central cornea were compared with hemolytic activities in the peripheral cornea for each of the following complement components : C1 , C4 , C2 , C3 , C5 , C6 , and C7 .
	manualset3
84779	1	398232	5	NULL	NULL	0	NULL	Hemophilia A ( HA )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemophilia A ( HA ) is caused by mutation in factor VIII ( FVIII ) gene in humans ; it leads to inadequate synthesis of active protein .
	manualset3
84780	2	398232	5	NULL	NULL	0	NULL	mutation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemophilia A ( HA ) is caused by mutation in factor VIII ( FVIII ) gene in humans ; it leads to inadequate synthesis of active protein .
	manualset3
84781	3	398232	5	NULL	NULL	0	NULL	factor VIII ( FVIII ) gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemophilia A ( HA ) is caused by mutation in factor VIII ( FVIII ) gene in humans ; it leads to inadequate synthesis of active protein .
	manualset3
84782	4	398232	5	NULL	NULL	0	NULL	humans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemophilia A ( HA ) is caused by mutation in factor VIII ( FVIII ) gene in humans ; it leads to inadequate synthesis of active protein .
	manualset3
84783	5	398232	5	NULL	NULL	0	NULL	inadequate synthesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemophilia A ( HA ) is caused by mutation in factor VIII ( FVIII ) gene in humans ; it leads to inadequate synthesis of active protein .
	manualset3
84784	6	398232	5	NULL	NULL	0	NULL	active protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemophilia A ( HA ) is caused by mutation in factor VIII ( FVIII ) gene in humans ; it leads to inadequate synthesis of active protein .
	manualset3
84785	1	398233	5	NULL	NULL	0	NULL	autopsy case	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( An autopsy case of lung cancer accompanied by pneumoperitoneum ) .
	manualset3
84786	2	398233	5	NULL	NULL	0	NULL	lung cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( An autopsy case of lung cancer accompanied by pneumoperitoneum ) .
	manualset3
84787	3	398233	5	NULL	NULL	0	NULL	pneumoperitoneum	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( An autopsy case of lung cancer accompanied by pneumoperitoneum ) .
	manualset3
84788	1	398234	5	NULL	NULL	0	NULL	Study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Study of influenza infection in organ cultures of human embryonic trachea ) .
	manualset3
84789	2	398234	5	NULL	NULL	0	NULL	influenza infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Study of influenza infection in organ cultures of human embryonic trachea ) .
	manualset3
84790	3	398234	5	NULL	NULL	0	NULL	organ cultures of human embryonic trachea	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Study of influenza infection in organ cultures of human embryonic trachea ) .
	manualset3
84791	1	398235	5	NULL	NULL	0	NULL	Hemorrhage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemorrhage is not as severe as in patients with hemophilia A or B. Data are presented suggesting that hemorrhage may , in part , be associated with aspirin use .
	manualset3
84792	2	398235	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemorrhage is not as severe as in patients with hemophilia A or B. Data are presented suggesting that hemorrhage may , in part , be associated with aspirin use .
	manualset3
84793	3	398235	5	NULL	NULL	0	NULL	hemophilia A or B	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemorrhage is not as severe as in patients with hemophilia A or B. Data are presented suggesting that hemorrhage may , in part , be associated with aspirin use .
	manualset3
84794	4	398235	5	NULL	NULL	0	NULL	Data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemorrhage is not as severe as in patients with hemophilia A or B. Data are presented suggesting that hemorrhage may , in part , be associated with aspirin use .
	manualset3
84795	5	398235	5	NULL	NULL	0	NULL	hemorrhage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemorrhage is not as severe as in patients with hemophilia A or B. Data are presented suggesting that hemorrhage may , in part , be associated with aspirin use .
	manualset3
84796	6	398235	5	NULL	NULL	NULL	NULL	aspirin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hemorrhage is not as severe as in patients with hemophilia A or B. Data are presented suggesting that hemorrhage may , in part , be associated with aspirin use .
	manualset3
84797	1	398236	5	NULL	NULL	0	NULL	Hemorrhagic complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemorrhagic complications in patients treated with anticoagulant doses of a low molecular weight heparin ( enoxaparin ) in routine hospital practice .
	manualset3
84798	2	398236	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemorrhagic complications in patients treated with anticoagulant doses of a low molecular weight heparin ( enoxaparin ) in routine hospital practice .
	manualset3
84799	3	398236	5	NULL	NULL	NULL	NULL	anticoagulant doses	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hemorrhagic complications in patients treated with anticoagulant doses of a low molecular weight heparin ( enoxaparin ) in routine hospital practice .
	manualset3
84800	5	398236	5	NULL	NULL	NULL	NULL	routine hospital practice	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hemorrhagic complications in patients treated with anticoagulant doses of a low molecular weight heparin ( enoxaparin ) in routine hospital practice .
	manualset3
84801	4	398236	5	NULL	NULL	0	NULL	low molecular weight heparin ( enoxaparin )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemorrhagic complications in patients treated with anticoagulant doses of a low molecular weight heparin ( enoxaparin ) in routine hospital practice .
	manualset3
84802	1	398237	5	NULL	NULL	0	NULL	Hemorrhagic cystitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemorrhagic cystitis can occur 6 months to 10 years after pelvic irradiation .
	manualset3
84803	2	398237	5	NULL	NULL	0	NULL	6 months to 10 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemorrhagic cystitis can occur 6 months to 10 years after pelvic irradiation .
	manualset3
84804	3	398237	5	NULL	NULL	0	NULL	pelvic irradiation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemorrhagic cystitis can occur 6 months to 10 years after pelvic irradiation .
	manualset3
84805	1	398238	5	NULL	NULL	0	NULL	Hemorrhagic lumbar synovial facet cyst	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemorrhagic lumbar synovial facet cyst secondary to anticoagulation therapy .
	manualset3
84806	2	398238	5	NULL	NULL	0	NULL	anticoagulation therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemorrhagic lumbar synovial facet cyst secondary to anticoagulation therapy .
	manualset3
84807	1	398239	5	NULL	NULL	0	NULL	Hemorrhagic shock	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemorrhagic shock renders patients susceptible to the development of acute lung injury in response to a second inflammatory stimulus by as yet unclear mechanisms .
	manualset3
84808	2	398239	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemorrhagic shock renders patients susceptible to the development of acute lung injury in response to a second inflammatory stimulus by as yet unclear mechanisms .
	manualset3
84809	3	398239	5	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemorrhagic shock renders patients susceptible to the development of acute lung injury in response to a second inflammatory stimulus by as yet unclear mechanisms .
	manualset3
84810	4	398239	5	NULL	NULL	0	NULL	acute lung injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemorrhagic shock renders patients susceptible to the development of acute lung injury in response to a second inflammatory stimulus by as yet unclear mechanisms .
	manualset3
84811	5	398239	5	NULL	NULL	0	NULL	response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemorrhagic shock renders patients susceptible to the development of acute lung injury in response to a second inflammatory stimulus by as yet unclear mechanisms .
	manualset3
84812	6	398239	5	NULL	NULL	0	NULL	second inflammatory stimulus	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemorrhagic shock renders patients susceptible to the development of acute lung injury in response to a second inflammatory stimulus by as yet unclear mechanisms .
	manualset3
84813	7	398239	5	NULL	NULL	0	NULL	unclear mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemorrhagic shock renders patients susceptible to the development of acute lung injury in response to a second inflammatory stimulus by as yet unclear mechanisms .
	manualset3
84814	1	398240	5	NULL	NULL	0	NULL	EFhd2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hence , EFhd2 regulates the BCR-elicited calcium flux through a calcium-dependent positive feedback mechanism in WEHI231 cells .
	manualset3
84815	2	398240	5	NULL	NULL	0	NULL	BCR-elicited calcium flux	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hence , EFhd2 regulates the BCR-elicited calcium flux through a calcium-dependent positive feedback mechanism in WEHI231 cells .
	manualset3
84816	3	398240	5	NULL	NULL	0	NULL	calcium-dependent positive feedback mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hence , EFhd2 regulates the BCR-elicited calcium flux through a calcium-dependent positive feedback mechanism in WEHI231 cells .
	manualset3
84817	4	398240	5	NULL	NULL	0	NULL	WEHI231 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Hence , EFhd2 regulates the BCR-elicited calcium flux through a calcium-dependent positive feedback mechanism in WEHI231 cells .
	manualset3
84818	1	398241	5	NULL	NULL	NULL	NULL	TRAIL-agonist compounds	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hence , TRAIL-agonist compounds have the potential of being excellent cancer therapeutic agents with minimal cytotoxicity .
	manualset3
84819	2	398241	5	NULL	NULL	NULL	NULL	excellent cancer therapeutic agents	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hence , TRAIL-agonist compounds have the potential of being excellent cancer therapeutic agents with minimal cytotoxicity .
	manualset3
84820	3	398241	5	NULL	NULL	0	NULL	minimal cytotoxicity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hence , TRAIL-agonist compounds have the potential of being excellent cancer therapeutic agents with minimal cytotoxicity .
	manualset3
84821	1	398242	5	NULL	NULL	NULL	NULL	compounds	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hence , compounds that bind phosphorus in the bowel are often necessary .
	manualset3
84822	2	398242	5	NULL	NULL	0	NULL	bind	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hence , compounds that bind phosphorus in the bowel are often necessary .
	manualset3
84823	3	398242	5	NULL	NULL	0	NULL	phosphorus	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Hence , compounds that bind phosphorus in the bowel are often necessary .
	manualset3
84824	4	398242	5	NULL	NULL	0	NULL	bowel	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Hence , compounds that bind phosphorus in the bowel are often necessary .
	manualset3
84825	1	398243	5	NULL	NULL	0	NULL	Study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Study of the factors responsible for the etiology of pressure sores ) .
	manualset3
84826	2	398243	5	NULL	NULL	0	NULL	 factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Study of the factors responsible for the etiology of pressure sores ) .
	manualset3
84827	3	398243	5	NULL	NULL	0	NULL	etiology	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Study of the factors responsible for the etiology of pressure sores ) .
	manualset3
84828	4	398243	5	NULL	NULL	0	NULL	pressure sores	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Study of the factors responsible for the etiology of pressure sores ) .
	manualset3
84829	1	398244	5	NULL	NULL	0	NULL	inadequate sleep	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hence , inadequate sleep is associated with development of obesity .
	manualset3
84830	2	398244	5	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hence , inadequate sleep is associated with development of obesity .
	manualset3
84831	3	398244	5	NULL	NULL	0	NULL	obesity	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hence , inadequate sleep is associated with development of obesity .
	manualset3
84832	1	398245	5	NULL	NULL	0	NULL	suppression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hence , suppression of glial proinflammatory responses can significantly reduce opioid withdrawal , while improving analgesia .
	manualset3
84833	2	398245	5	NULL	NULL	0	NULL	glial proinflammatory responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hence , suppression of glial proinflammatory responses can significantly reduce opioid withdrawal , while improving analgesia .
	manualset3
84834	3	398245	5	NULL	NULL	NULL	NULL	opioid withdrawal	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hence , suppression of glial proinflammatory responses can significantly reduce opioid withdrawal , while improving analgesia .
	manualset3
84835	4	398245	5	NULL	NULL	NULL	NULL	analgesia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hence , suppression of glial proinflammatory responses can significantly reduce opioid withdrawal , while improving analgesia .
	manualset3
84836	1	398246	5	NULL	NULL	0	NULL	 low-affinity A2A agonists CVT-3146 and CVT-3033	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Hence , the low-affinity A2A agonists CVT-3146 and CVT-3033 may prove to be superior to currently available high-affinity agonists as coronary vasodilators during myocardial imaging with radionuclide agents .
	manualset3
84837	2	398246	5	NULL	NULL	0	NULL	currently available high-affinity agonists	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Hence , the low-affinity A2A agonists CVT-3146 and CVT-3033 may prove to be superior to currently available high-affinity agonists as coronary vasodilators during myocardial imaging with radionuclide agents .
	manualset3
84838	3	398246	5	NULL	NULL	0	NULL	coronary vasodilators	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Hence , the low-affinity A2A agonists CVT-3146 and CVT-3033 may prove to be superior to currently available high-affinity agonists as coronary vasodilators during myocardial imaging with radionuclide agents .
	manualset3
84839	4	398246	5	NULL	NULL	0	NULL	myocardial imaging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hence , the low-affinity A2A agonists CVT-3146 and CVT-3033 may prove to be superior to currently available high-affinity agonists as coronary vasodilators during myocardial imaging with radionuclide agents .
	manualset3
84840	5	398246	5	NULL	NULL	0	NULL	radionuclide agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hence , the low-affinity A2A agonists CVT-3146 and CVT-3033 may prove to be superior to currently available high-affinity agonists as coronary vasodilators during myocardial imaging with radionuclide agents .
	manualset3
84841	1	398247	5	NULL	NULL	0	NULL	senile myoclonic epilepsy of Genton	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hence , the senile myoclonic epilepsy of Genton is an easily recognizable newer epileptic syndrome of the older Down syndrome patient .
	manualset3
84842	2	398247	5	NULL	NULL	0	NULL	epileptic syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hence , the senile myoclonic epilepsy of Genton is an easily recognizable newer epileptic syndrome of the older Down syndrome patient .
	manualset3
84843	3	398247	5	NULL	NULL	0	NULL	older Down syndrome patient	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hence , the senile myoclonic epilepsy of Genton is an easily recognizable newer epileptic syndrome of the older Down syndrome patient .
	manualset3
84844	1	398248	5	NULL	NULL	NULL	NULL	warfarin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hence , warfarin is significantly underused in clinical practice , with only half of warfarin-treated patients actually achieving therapeutic anticoagulation in routine clinical practice .
	manualset3
84845	2	398248	5	NULL	NULL	0	NULL	clinical practice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hence , warfarin is significantly underused in clinical practice , with only half of warfarin-treated patients actually achieving therapeutic anticoagulation in routine clinical practice .
	manualset3
84846	3	398248	5	NULL	NULL	0	NULL	warfarin-treated patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hence , warfarin is significantly underused in clinical practice , with only half of warfarin-treated patients actually achieving therapeutic anticoagulation in routine clinical practice .
	manualset3
84847	4	398248	5	NULL	NULL	0	NULL	therapeutic anticoagulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hence , warfarin is significantly underused in clinical practice , with only half of warfarin-treated patients actually achieving therapeutic anticoagulation in routine clinical practice .
	manualset3
84848	5	398248	5	NULL	NULL	0	NULL	routine clinical practice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hence , warfarin is significantly underused in clinical practice , with only half of warfarin-treated patients actually achieving therapeutic anticoagulation in routine clinical practice .
	manualset3
84849	1	398249	5	NULL	NULL	0	NULL	Heparin affinity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heparin affinity of factor VIIa : implications on the physiological inhibition by antithrombin and clearance of recombinant factor VIIa .
	manualset3
84850	2	398249	5	NULL	NULL	0	NULL	factor VIIa	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Heparin affinity of factor VIIa : implications on the physiological inhibition by antithrombin and clearance of recombinant factor VIIa .
	manualset3
84851	3	398249	5	NULL	NULL	0	NULL	implications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Heparin affinity of factor VIIa : implications on the physiological inhibition by antithrombin and clearance of recombinant factor VIIa .
	manualset3
84852	4	398249	5	NULL	NULL	0	NULL	physiological inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heparin affinity of factor VIIa : implications on the physiological inhibition by antithrombin and clearance of recombinant factor VIIa .
	manualset3
84853	5	398249	5	NULL	NULL	0	NULL	antithrombin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Heparin affinity of factor VIIa : implications on the physiological inhibition by antithrombin and clearance of recombinant factor VIIa .
	manualset3
84854	6	398249	5	NULL	NULL	0	NULL	clearance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heparin affinity of factor VIIa : implications on the physiological inhibition by antithrombin and clearance of recombinant factor VIIa .
	manualset3
84855	7	398249	5	NULL	NULL	0	NULL	recombinant factor VIIa	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Heparin affinity of factor VIIa : implications on the physiological inhibition by antithrombin and clearance of recombinant factor VIIa .
	manualset3
84856	1	398250	5	NULL	NULL	0	NULL	Heparin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Heparin and nitric oxide ( NO ) attenuate changes to the pulmonary vasculature caused by prolonged hypoxia .
	manualset3
84857	2	398250	5	NULL	NULL	0	NULL	nitric oxide ( NO )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Heparin and nitric oxide ( NO ) attenuate changes to the pulmonary vasculature caused by prolonged hypoxia .
	manualset3
84858	3	398250	5	NULL	NULL	0	NULL	pulmonary vasculature	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heparin and nitric oxide ( NO ) attenuate changes to the pulmonary vasculature caused by prolonged hypoxia .
	manualset3
84859	4	398250	5	NULL	NULL	0	NULL	prolonged hypoxia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Heparin and nitric oxide ( NO ) attenuate changes to the pulmonary vasculature caused by prolonged hypoxia .
	manualset3
84860	1	398251	5	NULL	NULL	NULL	NULL	Heparin and suramin treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Heparin and suramin treatment of these advanced embryos ( stage 4 ) revealed a dose-dependent inhibition on the regression of Hensen 's node and formation of mesodermal derivatives such as somites .
	manualset3
84861	2	398251	5	NULL	NULL	0	NULL	advanced embryos ( stage 4 )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Heparin and suramin treatment of these advanced embryos ( stage 4 ) revealed a dose-dependent inhibition on the regression of Hensen 's node and formation of mesodermal derivatives such as somites .
	manualset3
84862	3	398251	5	NULL	NULL	0	NULL	dose-dependent inhibition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Heparin and suramin treatment of these advanced embryos ( stage 4 ) revealed a dose-dependent inhibition on the regression of Hensen 's node and formation of mesodermal derivatives such as somites .
	manualset3
84863	4	398251	5	NULL	NULL	0	NULL	regression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heparin and suramin treatment of these advanced embryos ( stage 4 ) revealed a dose-dependent inhibition on the regression of Hensen 's node and formation of mesodermal derivatives such as somites .
	manualset3
84864	5	398251	5	NULL	NULL	0	NULL	Hensen 's node	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Heparin and suramin treatment of these advanced embryos ( stage 4 ) revealed a dose-dependent inhibition on the regression of Hensen 's node and formation of mesodermal derivatives such as somites .
	manualset3
84865	6	398251	5	NULL	NULL	0	NULL	formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heparin and suramin treatment of these advanced embryos ( stage 4 ) revealed a dose-dependent inhibition on the regression of Hensen 's node and formation of mesodermal derivatives such as somites .
	manualset3
84866	7	398251	5	NULL	NULL	NULL	NULL	mesodermal derivatives	AnatomicalPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Heparin and suramin treatment of these advanced embryos ( stage 4 ) revealed a dose-dependent inhibition on the regression of Hensen 's node and formation of mesodermal derivatives such as somites .
	manualset3
85498	8	398251	5	NULL	NULL	0	NULL	somites	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Heparin and suramin treatment of these advanced embryos ( stage 4 ) revealed a dose-dependent inhibition on the regression of Hensen 's node and formation of mesodermal derivatives such as somites .
	manualset3
84867	1	398252	5	NULL	NULL	NULL	NULL	Heparin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Heparin as an anti-inflammatory agent : it 's no GAG to forget about chemokines .
	manualset3
84868	2	398252	5	NULL	NULL	NULL	NULL	anti-inflammatory agent	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Heparin as an anti-inflammatory agent : it 's no GAG to forget about chemokines .
	manualset3
84869	3	398252	5	NULL	NULL	0	NULL	GAG	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Heparin as an anti-inflammatory agent : it 's no GAG to forget about chemokines .
	manualset3
84870	4	398252	5	NULL	NULL	0	NULL	chemokines	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Heparin as an anti-inflammatory agent : it 's no GAG to forget about chemokines .
	manualset3
84871	1	398253	5	NULL	NULL	0	NULL	 LDL receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Study on LDL receptors of liver non-parenchymal cells in hypertriglyceridemic rats induced by high carbohydrate diet ) .
	manualset3
84872	2	398253	5	NULL	NULL	0	NULL	liver non-parenchymal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	( Study on LDL receptors of liver non-parenchymal cells in hypertriglyceridemic rats induced by high carbohydrate diet ) .
	manualset3
84873	3	398253	5	NULL	NULL	0	NULL	hypertriglyceridemic rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Study on LDL receptors of liver non-parenchymal cells in hypertriglyceridemic rats induced by high carbohydrate diet ) .
	manualset3
84874	4	398253	5	NULL	NULL	0	NULL	high carbohydrate diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	( Study on LDL receptors of liver non-parenchymal cells in hypertriglyceridemic rats induced by high carbohydrate diet ) .
	manualset3
84875	1	398254	5	NULL	NULL	0	NULL	Heparin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Heparin inhibits the HDLp binding , indicating that positively charged groups are involved in the HDLp-fat body interaction .
	manualset3
84923	2	398254	5	NULL	NULL	0	NULL	HDLp	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Heparin inhibits the HDLp binding , indicating that positively charged groups are involved in the HDLp-fat body interaction .
	manualset3
84924	3	398254	5	NULL	NULL	0	NULL	positively charged groups	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Heparin inhibits the HDLp binding , indicating that positively charged groups are involved in the HDLp-fat body interaction .
	manualset3
84925	4	398254	5	NULL	NULL	0	NULL	HDLp-fat body interaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heparin inhibits the HDLp binding , indicating that positively charged groups are involved in the HDLp-fat body interaction .
	manualset3
84926	1	398255	5	NULL	NULL	0	NULL	Heparin levels	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Heparin levels may be used as an alternative for heparin monitoring but plasma levels of argatroban are not commercially available .
	manualset3
84927	2	398255	5	NULL	NULL	0	NULL	heparin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Heparin levels may be used as an alternative for heparin monitoring but plasma levels of argatroban are not commercially available .
	manualset3
84928	3	398255	5	NULL	NULL	0	NULL	plasma levels	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Heparin levels may be used as an alternative for heparin monitoring but plasma levels of argatroban are not commercially available .
	manualset3
84929	4	398255	5	NULL	NULL	0	NULL	argatroban	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Heparin levels may be used as an alternative for heparin monitoring but plasma levels of argatroban are not commercially available .
	manualset3
84930	1	398256	5	NULL	NULL	0	NULL	Hepatic Cd accumulation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatic Cd accumulation was linked to decreased cco-1 and sod-1 gene expression , whereas Cu accumulation was associated with a decrease in CCO enzymatic activity and an increase in total protein concentration and in cco-1 , mts and hsp-70 gene expression levels .
	manualset3
84931	2	398256	5	NULL	NULL	0	NULL	decreased cco-1 and sod-1 gene expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatic Cd accumulation was linked to decreased cco-1 and sod-1 gene expression , whereas Cu accumulation was associated with a decrease in CCO enzymatic activity and an increase in total protein concentration and in cco-1 , mts and hsp-70 gene expression levels .
	manualset3
84932	3	398256	5	NULL	NULL	NULL	NULL	Cu accumulation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hepatic Cd accumulation was linked to decreased cco-1 and sod-1 gene expression , whereas Cu accumulation was associated with a decrease in CCO enzymatic activity and an increase in total protein concentration and in cco-1 , mts and hsp-70 gene expression levels .
	manualset3
84933	4	398256	5	NULL	NULL	0	NULL	CCO enzymatic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatic Cd accumulation was linked to decreased cco-1 and sod-1 gene expression , whereas Cu accumulation was associated with a decrease in CCO enzymatic activity and an increase in total protein concentration and in cco-1 , mts and hsp-70 gene expression levels .
	manualset3
84934	5	398256	5	NULL	NULL	0	NULL	total protein concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatic Cd accumulation was linked to decreased cco-1 and sod-1 gene expression , whereas Cu accumulation was associated with a decrease in CCO enzymatic activity and an increase in total protein concentration and in cco-1 , mts and hsp-70 gene expression levels .
	manualset3
84935	6	398256	5	NULL	NULL	0	NULL	cco-1 , mts and hsp-70 gene expression levels	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatic Cd accumulation was linked to decreased cco-1 and sod-1 gene expression , whereas Cu accumulation was associated with a decrease in CCO enzymatic activity and an increase in total protein concentration and in cco-1 , mts and hsp-70 gene expression levels .
	manualset3
84936	1	398257	5	NULL	NULL	0	NULL	Hepatic abscess	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatic abscess presenting as severe fatigue and anemia .
	manualset3
84937	2	398257	5	NULL	NULL	0	NULL	severe fatigue	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatic abscess presenting as severe fatigue and anemia .
	manualset3
84938	3	398257	5	NULL	NULL	0	NULL	anemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatic abscess presenting as severe fatigue and anemia .
	manualset3
84939	1	398258	5	NULL	NULL	0	NULL	Hepatic iron loading	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatic iron loading in patients with compound heterozygous HFE mutations .
	manualset3
84940	2	398258	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatic iron loading in patients with compound heterozygous HFE mutations .
	manualset3
84941	3	398258	5	NULL	NULL	0	NULL	compound heterozygous HFE mutations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatic iron loading in patients with compound heterozygous HFE mutations .
	manualset3
84942	1	398259	5	NULL	NULL	0	NULL	Hepatic lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatic lesions and bacterial changes in mice during infection of Fusobacterium necrophorum .
	manualset3
84943	2	398259	5	NULL	NULL	0	NULL	bacterial changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatic lesions and bacterial changes in mice during infection of Fusobacterium necrophorum .
	manualset3
84944	3	398259	5	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatic lesions and bacterial changes in mice during infection of Fusobacterium necrophorum .
	manualset3
84945	4	398259	5	NULL	NULL	NULL	NULL	infection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hepatic lesions and bacterial changes in mice during infection of Fusobacterium necrophorum .
	manualset3
84946	5	398259	5	NULL	NULL	0	NULL	Fusobacterium necrophorum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatic lesions and bacterial changes in mice during infection of Fusobacterium necrophorum .
	manualset3
84947	1	398260	5	NULL	NULL	0	NULL	Study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Study on linkage between polymorphism of interleukin 6 gene -572 C/G and susceptibility to myocardial infarction ) .
	manualset3
84948	2	398260	5	NULL	NULL	0	NULL	linkage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Study on linkage between polymorphism of interleukin 6 gene -572 C/G and susceptibility to myocardial infarction ) .
	manualset3
84949	3	398260	5	NULL	NULL	0	NULL	polymorphism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Study on linkage between polymorphism of interleukin 6 gene -572 C/G and susceptibility to myocardial infarction ) .
	manualset3
84950	4	398260	5	NULL	NULL	0	NULL	interleukin 6 gene -572 C/G	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	( Study on linkage between polymorphism of interleukin 6 gene -572 C/G and susceptibility to myocardial infarction ) .
	manualset3
84951	5	398260	5	NULL	NULL	0	NULL	susceptibility	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Study on linkage between polymorphism of interleukin 6 gene -572 C/G and susceptibility to myocardial infarction ) .
	manualset3
84952	6	398260	5	NULL	NULL	0	NULL	myocardial infarction	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Study on linkage between polymorphism of interleukin 6 gene -572 C/G and susceptibility to myocardial infarction ) .
	manualset3
84953	1	398261	5	NULL	NULL	0	NULL	Hepatic stellate cells ( HpSTCs )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatic stellate cells ( HpSTCs ) are major regulators of hepatic fibrogenesis in adults .
	manualset3
84954	2	398261	5	NULL	NULL	0	NULL	major regulators	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatic stellate cells ( HpSTCs ) are major regulators of hepatic fibrogenesis in adults .
	manualset3
84955	3	398261	5	NULL	NULL	0	NULL	hepatic fibrogenesis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatic stellate cells ( HpSTCs ) are major regulators of hepatic fibrogenesis in adults .
	manualset3
84956	4	398261	5	NULL	NULL	0	NULL	adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatic stellate cells ( HpSTCs ) are major regulators of hepatic fibrogenesis in adults .
	manualset3
84957	1	398262	5	NULL	NULL	0	NULL	Hepatitis B virus ( HBV ) infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatitis B virus ( HBV ) infection , one of the major health priorities , accounts approximately for 350 million chronic cases and a global total of 33 million people were living with human immunodeficiency virus ( HIV ) in the world.Co-infection with HIV and the HBV presents a significant challenge to health care providers , with different prevalence rates in different parts of the world .
	manualset3
84958	3	398262	5	NULL	NULL	NULL	NULL	350 million chronic cases	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hepatitis B virus ( HBV ) infection , one of the major health priorities , accounts approximately for 350 million chronic cases and a global total of 33 million people were living with human immunodeficiency virus ( HIV ) in the world.Co-infection with HIV and the HBV presents a significant challenge to health care providers , with different prevalence rates in different parts of the world .
	manualset3
84959	4	398262	5	NULL	NULL	NULL	NULL	33 million people	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hepatitis B virus ( HBV ) infection , one of the major health priorities , accounts approximately for 350 million chronic cases and a global total of 33 million people were living with human immunodeficiency virus ( HIV ) in the world.Co-infection with HIV and the HBV presents a significant challenge to health care providers , with different prevalence rates in different parts of the world .
	manualset3
84960	5	398262	5	NULL	NULL	NULL	NULL	human immunodeficiency virus ( HIV )	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hepatitis B virus ( HBV ) infection , one of the major health priorities , accounts approximately for 350 million chronic cases and a global total of 33 million people were living with human immunodeficiency virus ( HIV ) in the world.Co-infection with HIV and the HBV presents a significant challenge to health care providers , with different prevalence rates in different parts of the world .
	manualset3
84961	6	398262	5	NULL	NULL	NULL	NULL	world	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hepatitis B virus ( HBV ) infection , one of the major health priorities , accounts approximately for 350 million chronic cases and a global total of 33 million people were living with human immunodeficiency virus ( HIV ) in the world.Co-infection with HIV and the HBV presents a significant challenge to health care providers , with different prevalence rates in different parts of the world .
	manualset3
84962	7	398262	5	NULL	NULL	NULL	NULL	Co-infection with HIV and the HBV	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hepatitis B virus ( HBV ) infection , one of the major health priorities , accounts approximately for 350 million chronic cases and a global total of 33 million people were living with human immunodeficiency virus ( HIV ) in the world.Co-infection with HIV and the HBV presents a significant challenge to health care providers , with different prevalence rates in different parts of the world .
	manualset3
84965	8	398262	5	NULL	NULL	NULL	NULL	health care providers	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hepatitis B virus ( HBV ) infection , one of the major health priorities , accounts approximately for 350 million chronic cases and a global total of 33 million people were living with human immunodeficiency virus ( HIV ) in the world.Co-infection with HIV and the HBV presents a significant challenge to health care providers , with different prevalence rates in different parts of the world .
	manualset3
84967	9	398262	5	NULL	NULL	NULL	NULL	different parts of the world	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hepatitis B virus ( HBV ) infection , one of the major health priorities , accounts approximately for 350 million chronic cases and a global total of 33 million people were living with human immunodeficiency virus ( HIV ) in the world.Co-infection with HIV and the HBV presents a significant challenge to health care providers , with different prevalence rates in different parts of the world .
	manualset3
85433	2	398262	5	NULL	NULL	0	NULL	major health priorities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatitis B virus ( HBV ) infection , one of the major health priorities , accounts approximately for 350 million chronic cases and a global total of 33 million people were living with human immunodeficiency virus ( HIV ) in the world.Co-infection with HIV and the HBV presents a significant challenge to health care providers , with different prevalence rates in different parts of the world .
	manualset3
84969	1	398263	5	NULL	NULL	0	NULL	Hepatitis B virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatitis B virus alters the antioxidant system in transgenic mice and sensitizes hepatocytes to Fas signaling .
	manualset3
84970	2	398263	5	NULL	NULL	0	NULL	antioxidant system	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatitis B virus alters the antioxidant system in transgenic mice and sensitizes hepatocytes to Fas signaling .
	manualset3
84971	3	398263	5	NULL	NULL	0	NULL	transgenic mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatitis B virus alters the antioxidant system in transgenic mice and sensitizes hepatocytes to Fas signaling .
	manualset3
84972	4	398263	5	NULL	NULL	0	NULL	hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatitis B virus alters the antioxidant system in transgenic mice and sensitizes hepatocytes to Fas signaling .
	manualset3
84973	5	398263	5	NULL	NULL	0	NULL	Fas signaling	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatitis B virus alters the antioxidant system in transgenic mice and sensitizes hepatocytes to Fas signaling .
	manualset3
84974	1	398264	5	NULL	NULL	NULL	NULL	Hepatitis C prevalence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hepatitis C prevalence and needle/syringe sharing behaviors in recent onset injecting drug users .
	manualset3
84975	2	398264	5	NULL	NULL	0	NULL	needle/syringe sharing behaviors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatitis C prevalence and needle/syringe sharing behaviors in recent onset injecting drug users .
	manualset3
84976	3	398264	5	NULL	NULL	0	NULL	drug users	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatitis C prevalence and needle/syringe sharing behaviors in recent onset injecting drug users .
	manualset3
84977	1	398265	5	NULL	NULL	0	NULL	Hepatitis C virus ( HCV )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatitis C virus ( HCV ) has a high propensity for persistence .
	manualset3
84978	2	398265	5	NULL	NULL	0	NULL	high propensity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatitis C virus ( HCV ) has a high propensity for persistence .
	manualset3
84979	3	398265	5	NULL	NULL	0	NULL	persistence 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatitis C virus ( HCV ) has a high propensity for persistence .
	manualset3
84980	1	398266	5	NULL	NULL	0	NULL	Hepatoblastoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatoblastoma , thrombocytosis , and increased thrombopoietin .
	manualset3
84981	2	398266	5	NULL	NULL	0	NULL	thrombocytosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatoblastoma , thrombocytosis , and increased thrombopoietin .
	manualset3
84982	3	398266	5	NULL	NULL	0	NULL	increased thrombopoietin	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatoblastoma , thrombocytosis , and increased thrombopoietin .
	manualset3
84983	1	398267	5	NULL	NULL	0	NULL	Hepatocellular necrosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatocellular necrosis , fibrosis and microsomal activity determine the hepatic pharmacokinetics of basic drugs in right-heart-failure-induced liver damage .
	manualset3
84984	2	398267	5	NULL	NULL	0	NULL	fibrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatocellular necrosis , fibrosis and microsomal activity determine the hepatic pharmacokinetics of basic drugs in right-heart-failure-induced liver damage .
	manualset3
84985	3	398267	5	NULL	NULL	0	NULL	microsomal activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatocellular necrosis , fibrosis and microsomal activity determine the hepatic pharmacokinetics of basic drugs in right-heart-failure-induced liver damage .
	manualset3
84986	4	398267	5	NULL	NULL	0	NULL	hepatic pharmacokinetics	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatocellular necrosis , fibrosis and microsomal activity determine the hepatic pharmacokinetics of basic drugs in right-heart-failure-induced liver damage .
	manualset3
84987	5	398267	5	NULL	NULL	NULL	NULL	basic drugs	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hepatocellular necrosis , fibrosis and microsomal activity determine the hepatic pharmacokinetics of basic drugs in right-heart-failure-induced liver damage .
	manualset3
84988	6	398267	5	NULL	NULL	0	NULL	right-heart-failure-induced liver damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatocellular necrosis , fibrosis and microsomal activity determine the hepatic pharmacokinetics of basic drugs in right-heart-failure-induced liver damage .
	manualset3
84989	1	398268	5	NULL	NULL	0	NULL	Hepatocyte-specific knockout	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatocyte-specific knockout of - catenin inhibited CAR agonists-induced hepatocyte proliferation in male mice .
	manualset3
84990	2	398268	5	NULL	NULL	0	NULL	catenin	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatocyte-specific knockout of - catenin inhibited CAR agonists-induced hepatocyte proliferation in male mice .
	manualset3
84991	3	398268	5	NULL	NULL	0	NULL	CAR agonists-induced hepatocyte proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatocyte-specific knockout of - catenin inhibited CAR agonists-induced hepatocyte proliferation in male mice .
	manualset3
84992	4	398268	5	NULL	NULL	0	NULL	male mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatocyte-specific knockout of - catenin inhibited CAR agonists-induced hepatocyte proliferation in male mice .
	manualset3
84993	1	398269	5	NULL	NULL	0	NULL	Hepatocyte nuclear factor 4 alpha ( HNF4 alpha )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatocyte nuclear factor 4 alpha ( HNF4 alpha ) is a member of the nuclear receptor superfamily and is expressed in several endodermal tissues .
	manualset3
84994	2	398269	5	NULL	NULL	0	NULL	nuclear receptor superfamily	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatocyte nuclear factor 4 alpha ( HNF4 alpha ) is a member of the nuclear receptor superfamily and is expressed in several endodermal tissues .
	manualset3
84995	3	398269	5	NULL	NULL	0	NULL	endodermal tissues	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatocyte nuclear factor 4 alpha ( HNF4 alpha ) is a member of the nuclear receptor superfamily and is expressed in several endodermal tissues .
	manualset3
84996	1	398270	5	NULL	NULL	0	NULL	Hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatocytes derived from embryonic stem cells ( ESCs ) are expected to be useful for basic research and clinical applications .
	manualset3
84997	2	398270	5	NULL	NULL	0	NULL	embryonic stem cells ( ESCs )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatocytes derived from embryonic stem cells ( ESCs ) are expected to be useful for basic research and clinical applications .
	manualset3
84998	3	398270	5	NULL	NULL	0	NULL	basic research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatocytes derived from embryonic stem cells ( ESCs ) are expected to be useful for basic research and clinical applications .
	manualset3
84999	4	398270	5	NULL	NULL	0	NULL	clinical applications	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatocytes derived from embryonic stem cells ( ESCs ) are expected to be useful for basic research and clinical applications .
	manualset3
85000	1	398271	5	NULL	NULL	0	NULL	Hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatocytes obtained from ( RHA ) Wistar rats by collagenase perfusion were seeded onto non-woven filamentous sheets of polyglycolic acid 1 x 3 cm in size and 2 mm thickness to a density of 500 , 000 cells/cm2 .
	manualset3
85001	2	398271	5	NULL	NULL	0	NULL	( RHA ) Wistar rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatocytes obtained from ( RHA ) Wistar rats by collagenase perfusion were seeded onto non-woven filamentous sheets of polyglycolic acid 1 x 3 cm in size and 2 mm thickness to a density of 500 , 000 cells/cm2 .
	manualset3
85002	3	398271	5	NULL	NULL	0	NULL	collagenase perfusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatocytes obtained from ( RHA ) Wistar rats by collagenase perfusion were seeded onto non-woven filamentous sheets of polyglycolic acid 1 x 3 cm in size and 2 mm thickness to a density of 500 , 000 cells/cm2 .
	manualset3
85003	4	398271	5	NULL	NULL	0	NULL	non-woven filamentous sheets	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatocytes obtained from ( RHA ) Wistar rats by collagenase perfusion were seeded onto non-woven filamentous sheets of polyglycolic acid 1 x 3 cm in size and 2 mm thickness to a density of 500 , 000 cells/cm2 .
	manualset3
85004	5	398271	5	NULL	NULL	0	NULL	polyglycolic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatocytes obtained from ( RHA ) Wistar rats by collagenase perfusion were seeded onto non-woven filamentous sheets of polyglycolic acid 1 x 3 cm in size and 2 mm thickness to a density of 500 , 000 cells/cm2 .
	manualset3
85005	6	398271	5	NULL	NULL	NULL	NULL	1 x 3 cm in size	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hepatocytes obtained from ( RHA ) Wistar rats by collagenase perfusion were seeded onto non-woven filamentous sheets of polyglycolic acid 1 x 3 cm in size and 2 mm thickness to a density of 500 , 000 cells/cm2 .
	manualset3
85006	7	398271	5	NULL	NULL	NULL	NULL	2 mm thickness	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hepatocytes obtained from ( RHA ) Wistar rats by collagenase perfusion were seeded onto non-woven filamentous sheets of polyglycolic acid 1 x 3 cm in size and 2 mm thickness to a density of 500 , 000 cells/cm2 .
	manualset3
85007	8	398271	5	NULL	NULL	NULL	NULL	density of 500 , 000 cells/cm2	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hepatocytes obtained from ( RHA ) Wistar rats by collagenase perfusion were seeded onto non-woven filamentous sheets of polyglycolic acid 1 x 3 cm in size and 2 mm thickness to a density of 500 , 000 cells/cm2 .
	manualset3
85008	1	398272	5	NULL	NULL	0	NULL	Hepatoma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatoma cells were infected with AdB17 or AdB17-beta with AdLacZ , an adenovirus expressing beta-galactosidase , as a control .
	manualset3
85412	2	398272	5	NULL	NULL	NULL	NULL	AdB17	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hepatoma cells were infected with AdB17 or AdB17-beta with AdLacZ , an adenovirus expressing beta-galactosidase , as a control .
	manualset3
85413	3	398272	5	NULL	NULL	0	NULL	AdB17-beta with AdLacZ	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatoma cells were infected with AdB17 or AdB17-beta with AdLacZ , an adenovirus expressing beta-galactosidase , as a control .
	manualset3
85414	4	398272	5	NULL	NULL	0	NULL	adenovirus expressing beta-galactosidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatoma cells were infected with AdB17 or AdB17-beta with AdLacZ , an adenovirus expressing beta-galactosidase , as a control .
	manualset3
85415	5	398272	5	NULL	NULL	NULL	NULL	control	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hepatoma cells were infected with AdB17 or AdB17-beta with AdLacZ , an adenovirus expressing beta-galactosidase , as a control .
	manualset3
85162	1	398273	5	NULL	NULL	0	NULL	Hepatoregenerative role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatoregenerative role of bone morphogenetic protein-9 .
	manualset3
85163	2	398273	5	NULL	NULL	0	NULL	bone morphogenetic protein-9	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatoregenerative role of bone morphogenetic protein-9 .
	manualset3
85164	1	398274	5	NULL	NULL	0	NULL	Hepatosplanchnic blood flow control	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatosplanchnic blood flow control and oxygen extraction are modified by the underlying mechanism of impaired perfusion .
	manualset3
85165	2	398274	5	NULL	NULL	0	NULL	oxygen extraction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatosplanchnic blood flow control and oxygen extraction are modified by the underlying mechanism of impaired perfusion .
	manualset3
85166	3	398274	5	NULL	NULL	0	NULL	underlying mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatosplanchnic blood flow control and oxygen extraction are modified by the underlying mechanism of impaired perfusion .
	manualset3
85167	4	398274	5	NULL	NULL	0	NULL	impaired perfusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatosplanchnic blood flow control and oxygen extraction are modified by the underlying mechanism of impaired perfusion .
	manualset3
85168	1	398275	5	NULL	NULL	0	NULL	Hepatosplenomegaly	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatosplenomegaly was diagnosed by USG examination .
	manualset3
85169	2	398275	5	NULL	NULL	0	NULL	USG examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatosplenomegaly was diagnosed by USG examination .
	manualset3
85170	1	398276	5	NULL	NULL	NULL	NULL	adrenal mass	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Her general condition has markedly improved and her adrenal mass and meningioma are being closely observed now .
	manualset3
85171	2	398276	5	NULL	NULL	0	NULL	meningioma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Her general condition has markedly improved and her adrenal mass and meningioma are being closely observed now .
	manualset3
85172	1	398277	5	NULL	NULL	NULL	NULL	hemoglobin level	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Her hemoglobin level was 8.3 g/dl .
	manualset3
85173	2	398277	5	NULL	NULL	0	NULL	8.3 g/dl	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Her hemoglobin level was 8.3 g/dl .
	manualset3
85174	1	398278	5	NULL	NULL	0	NULL	serum calcium level	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Her serum calcium level ranged from 9.0 to 10.0 mg/dL , which caused difficulties in performing vitamin D injection therapy .
	manualset3
85175	2	398278	5	NULL	NULL	0	NULL	9.0 to 10.0 mg/dL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Her serum calcium level ranged from 9.0 to 10.0 mg/dL , which caused difficulties in performing vitamin D injection therapy .
	manualset3
85176	3	398278	5	NULL	NULL	0	NULL	vitamin D injection therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Her serum calcium level ranged from 9.0 to 10.0 mg/dL , which caused difficulties in performing vitamin D injection therapy .
	manualset3
85177	1	398279	5	NULL	NULL	NULL	NULL	sister aged two months	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Her sister aged two months received porcine calcitonin for three weeks , during which clinical improvement , no change in the serum level of alkaline phosphatase and a marked decrease of the excretion of hydroxyproline were recorded .
	manualset3
85179	2	398279	5	NULL	NULL	NULL	NULL	porcine calcitonin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Her sister aged two months received porcine calcitonin for three weeks , during which clinical improvement , no change in the serum level of alkaline phosphatase and a marked decrease of the excretion of hydroxyproline were recorded .
	manualset3
85180	3	398279	5	NULL	NULL	NULL	NULL	three weeks	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Her sister aged two months received porcine calcitonin for three weeks , during which clinical improvement , no change in the serum level of alkaline phosphatase and a marked decrease of the excretion of hydroxyproline were recorded .
	manualset3
85181	4	398279	5	NULL	NULL	NULL	NULL	clinical improvement	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Her sister aged two months received porcine calcitonin for three weeks , during which clinical improvement , no change in the serum level of alkaline phosphatase and a marked decrease of the excretion of hydroxyproline were recorded .
	manualset3
85182	5	398279	5	NULL	NULL	NULL	NULL	serum level	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Her sister aged two months received porcine calcitonin for three weeks , during which clinical improvement , no change in the serum level of alkaline phosphatase and a marked decrease of the excretion of hydroxyproline were recorded .
	manualset3
85183	6	398279	5	NULL	NULL	NULL	NULL	alkaline phosphatase	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Her sister aged two months received porcine calcitonin for three weeks , during which clinical improvement , no change in the serum level of alkaline phosphatase and a marked decrease of the excretion of hydroxyproline were recorded .
	manualset3
85184	7	398279	5	NULL	NULL	NULL	NULL	excretion	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Her sister aged two months received porcine calcitonin for three weeks , during which clinical improvement , no change in the serum level of alkaline phosphatase and a marked decrease of the excretion of hydroxyproline were recorded .
	manualset3
85185	8	398279	5	NULL	NULL	NULL	NULL	hydroxyproline	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Her sister aged two months received porcine calcitonin for three weeks , during which clinical improvement , no change in the serum level of alkaline phosphatase and a marked decrease of the excretion of hydroxyproline were recorded .
	manualset3
85186	1	398280	5	NULL	NULL	0	NULL	purification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , I report a method that was originally designed for purification of large amounts of nucleotides using anion-exchanging resin but has shown the promise of enriching phosphorylated peptides .
	manualset3
85187	2	398280	5	NULL	NULL	0	NULL	nucleotides	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , I report a method that was originally designed for purification of large amounts of nucleotides using anion-exchanging resin but has shown the promise of enriching phosphorylated peptides .
	manualset3
85188	3	398280	5	NULL	NULL	0	NULL	anion-exchanging resin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , I report a method that was originally designed for purification of large amounts of nucleotides using anion-exchanging resin but has shown the promise of enriching phosphorylated peptides .
	manualset3
85189	4	398280	5	NULL	NULL	0	NULL	phosphorylated peptides	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , I report a method that was originally designed for purification of large amounts of nucleotides using anion-exchanging resin but has shown the promise of enriching phosphorylated peptides .
	manualset3
85190	1	398281	5	NULL	NULL	0	NULL	MRP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , MRP was detected in several types of epithelia , muscle cells , and macrophages .
	manualset3
85191	2	398281	5	NULL	NULL	0	NULL	epithelia	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , MRP was detected in several types of epithelia , muscle cells , and macrophages .
	manualset3
85192	3	398281	5	NULL	NULL	0	NULL	muscle cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , MRP was detected in several types of epithelia , muscle cells , and macrophages .
	manualset3
85193	4	398281	5	NULL	NULL	0	NULL	macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , MRP was detected in several types of epithelia , muscle cells , and macrophages .
	manualset3
85194	1	398282	5	NULL	NULL	0	NULL	metastatic renal cell carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , a case of metastatic renal cell carcinoma to muscle and jejunum is reported .
	manualset3
85195	2	398282	5	NULL	NULL	0	NULL	muscle	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , a case of metastatic renal cell carcinoma to muscle and jejunum is reported .
	manualset3
85196	3	398282	5	NULL	NULL	0	NULL	jejunum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , a case of metastatic renal cell carcinoma to muscle and jejunum is reported .
	manualset3
85197	1	398283	5	NULL	NULL	0	NULL	recent data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , based upon the recent data , mainly obtained from the DT40 system , we discuss several new aspects on mechanisms by which BCR signals are propagated and modified .
	manualset3
85198	2	398283	5	NULL	NULL	0	NULL	DT40 system	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , based upon the recent data , mainly obtained from the DT40 system , we discuss several new aspects on mechanisms by which BCR signals are propagated and modified .
	manualset3
85199	3	398283	5	NULL	NULL	0	NULL	BCR signals	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , based upon the recent data , mainly obtained from the DT40 system , we discuss several new aspects on mechanisms by which BCR signals are propagated and modified .
	manualset3
85200	1	398284	5	NULL	NULL	0	NULL	Subcutaneous traumatic gallbladder rupture	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Subcutaneous traumatic gallbladder rupture ) .
	manualset3
85416	1	398285	5	NULL	NULL	0	NULL	altimetry-derived variation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , for the first time , we have further used the altimetry-derived variation of water level for estimating the fluctuation of water storage as an addition to the present in situ water storage estimation systems to be used in remote areas and in emergency situation such as in the events flooding monitoring and for studying the effect of climate change .
	manualset3
85417	2	398285	5	NULL	NULL	0	NULL	water level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , for the first time , we have further used the altimetry-derived variation of water level for estimating the fluctuation of water storage as an addition to the present in situ water storage estimation systems to be used in remote areas and in emergency situation such as in the events flooding monitoring and for studying the effect of climate change .
	manualset3
85418	3	398285	5	NULL	NULL	0	NULL	fluctuation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , for the first time , we have further used the altimetry-derived variation of water level for estimating the fluctuation of water storage as an addition to the present in situ water storage estimation systems to be used in remote areas and in emergency situation such as in the events flooding monitoring and for studying the effect of climate change .
	manualset3
85419	4	398285	5	NULL	NULL	0	NULL	water storage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , for the first time , we have further used the altimetry-derived variation of water level for estimating the fluctuation of water storage as an addition to the present in situ water storage estimation systems to be used in remote areas and in emergency situation such as in the events flooding monitoring and for studying the effect of climate change .
	manualset3
85420	5	398285	5	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , for the first time , we have further used the altimetry-derived variation of water level for estimating the fluctuation of water storage as an addition to the present in situ water storage estimation systems to be used in remote areas and in emergency situation such as in the events flooding monitoring and for studying the effect of climate change .
	manualset3
85421	6	398285	5	NULL	NULL	0	NULL	situ water storage estimation systems	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , for the first time , we have further used the altimetry-derived variation of water level for estimating the fluctuation of water storage as an addition to the present in situ water storage estimation systems to be used in remote areas and in emergency situation such as in the events flooding monitoring and for studying the effect of climate change .
	manualset3
85422	7	398285	5	NULL	NULL	0	NULL	remote areas	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , for the first time , we have further used the altimetry-derived variation of water level for estimating the fluctuation of water storage as an addition to the present in situ water storage estimation systems to be used in remote areas and in emergency situation such as in the events flooding monitoring and for studying the effect of climate change .
	manualset3
85423	8	398285	5	NULL	NULL	0	NULL	emergency situation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , for the first time , we have further used the altimetry-derived variation of water level for estimating the fluctuation of water storage as an addition to the present in situ water storage estimation systems to be used in remote areas and in emergency situation such as in the events flooding monitoring and for studying the effect of climate change .
	manualset3
85424	9	398285	5	NULL	NULL	0	NULL	events flooding monitoring	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , for the first time , we have further used the altimetry-derived variation of water level for estimating the fluctuation of water storage as an addition to the present in situ water storage estimation systems to be used in remote areas and in emergency situation such as in the events flooding monitoring and for studying the effect of climate change .
	manualset3
85425	10	398285	5	NULL	NULL	0	NULL	climate change	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , for the first time , we have further used the altimetry-derived variation of water level for estimating the fluctuation of water storage as an addition to the present in situ water storage estimation systems to be used in remote areas and in emergency situation such as in the events flooding monitoring and for studying the effect of climate change .
	manualset3
85201	1	398286	5	NULL	NULL	0	NULL	scintigraphy	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , scintigraphy is superior to all other imaging procedures in the evaluation of bile flow situations .
	manualset3
85202	2	398286	5	NULL	NULL	0	NULL	imaging procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , scintigraphy is superior to all other imaging procedures in the evaluation of bile flow situations .
	manualset3
85203	3	398286	5	NULL	NULL	0	NULL	evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , scintigraphy is superior to all other imaging procedures in the evaluation of bile flow situations .
	manualset3
85204	4	398286	5	NULL	NULL	0	NULL	bile flow situations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , scintigraphy is superior to all other imaging procedures in the evaluation of bile flow situations .
	manualset3
85205	1	398287	5	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , the authors present a case of a drug-resistant epilepsy patient with a complex phenotype where a diagnosis of CTX was done and showed a significant reduction in seizure frequency after chenodeoxycholic acid supplementation .
	manualset3
85206	2	398287	5	NULL	NULL	0	NULL	case	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , the authors present a case of a drug-resistant epilepsy patient with a complex phenotype where a diagnosis of CTX was done and showed a significant reduction in seizure frequency after chenodeoxycholic acid supplementation .
	manualset3
85207	3	398287	5	NULL	NULL	0	NULL	drug-resistant epilepsy patient	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , the authors present a case of a drug-resistant epilepsy patient with a complex phenotype where a diagnosis of CTX was done and showed a significant reduction in seizure frequency after chenodeoxycholic acid supplementation .
	manualset3
85208	4	398287	5	NULL	NULL	0	NULL	complex phenotype	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , the authors present a case of a drug-resistant epilepsy patient with a complex phenotype where a diagnosis of CTX was done and showed a significant reduction in seizure frequency after chenodeoxycholic acid supplementation .
	manualset3
85209	5	398287	5	NULL	NULL	NULL	NULL	diagnosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , the authors present a case of a drug-resistant epilepsy patient with a complex phenotype where a diagnosis of CTX was done and showed a significant reduction in seizure frequency after chenodeoxycholic acid supplementation .
	manualset3
85210	6	398287	5	NULL	NULL	0	NULL	CTX	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , the authors present a case of a drug-resistant epilepsy patient with a complex phenotype where a diagnosis of CTX was done and showed a significant reduction in seizure frequency after chenodeoxycholic acid supplementation .
	manualset3
85211	7	398287	5	NULL	NULL	0	NULL	significant reduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , the authors present a case of a drug-resistant epilepsy patient with a complex phenotype where a diagnosis of CTX was done and showed a significant reduction in seizure frequency after chenodeoxycholic acid supplementation .
	manualset3
85212	8	398287	5	NULL	NULL	0	NULL	seizure frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , the authors present a case of a drug-resistant epilepsy patient with a complex phenotype where a diagnosis of CTX was done and showed a significant reduction in seizure frequency after chenodeoxycholic acid supplementation .
	manualset3
85213	9	398287	5	NULL	NULL	0	NULL	chenodeoxycholic acid supplementation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , the authors present a case of a drug-resistant epilepsy patient with a complex phenotype where a diagnosis of CTX was done and showed a significant reduction in seizure frequency after chenodeoxycholic acid supplementation .
	manualset3
85214	1	398288	5	NULL	NULL	NULL	NULL	oxygen concentration	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , the effects of oxygen concentration and temperature on the kinetic isotope effects with deuterated choline have been investigated .
	manualset3
85215	2	398288	5	NULL	NULL	0	NULL	temperature	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , the effects of oxygen concentration and temperature on the kinetic isotope effects with deuterated choline have been investigated .
	manualset3
85216	3	398288	5	NULL	NULL	0	NULL	kinetic isotope effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , the effects of oxygen concentration and temperature on the kinetic isotope effects with deuterated choline have been investigated .
	manualset3
85217	4	398288	5	NULL	NULL	0	NULL	deuterated choline	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , the effects of oxygen concentration and temperature on the kinetic isotope effects with deuterated choline have been investigated .
	manualset3
85218	1	398289	5	NULL	NULL	0	NULL	two genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , two genes are identified , ARE1 and ARE2 , that encode ACAT-related enzymes in yeast .
	manualset3
85219	2	398289	5	NULL	NULL	0	NULL	ARE1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , two genes are identified , ARE1 and ARE2 , that encode ACAT-related enzymes in yeast .
	manualset3
85220	3	398289	5	NULL	NULL	0	NULL	ARE2	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , two genes are identified , ARE1 and ARE2 , that encode ACAT-related enzymes in yeast .
	manualset3
85221	4	398289	5	NULL	NULL	0	NULL	encode	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , two genes are identified , ARE1 and ARE2 , that encode ACAT-related enzymes in yeast .
	manualset3
85222	5	398289	5	NULL	NULL	0	NULL	ACAT-related enzymes	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , two genes are identified , ARE1 and ARE2 , that encode ACAT-related enzymes in yeast .
	manualset3
85223	6	398289	5	NULL	NULL	0	NULL	yeast	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , two genes are identified , ARE1 and ARE2 , that encode ACAT-related enzymes in yeast .
	manualset3
85224	1	398290	5	NULL	NULL	0	NULL	viruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , viruses are detected using an immunoassay sandwich approach with the reporting antibodies tagged to liposomes .
	manualset3
85225	2	398290	5	NULL	NULL	0	NULL	immunoassay sandwich approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , viruses are detected using an immunoassay sandwich approach with the reporting antibodies tagged to liposomes .
	manualset3
85226	3	398290	5	NULL	NULL	0	NULL	reporting antibodies	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , viruses are detected using an immunoassay sandwich approach with the reporting antibodies tagged to liposomes .
	manualset3
85227	4	398290	5	NULL	NULL	0	NULL	liposomes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , viruses are detected using an immunoassay sandwich approach with the reporting antibodies tagged to liposomes .
	manualset3
85228	1	398291	5	NULL	NULL	NULL	NULL	constitutive monocyte TLR2 expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we analyzed constitutive monocyte TLR2 expression and evaluated the expression profiles of the proximal downstream adapter molecule myeloid differentiation factor 88 ( MyD88 ) .
	manualset3
85230	2	398291	5	NULL	NULL	NULL	NULL	proximal downstream adapter molecule myeloid differentiation factor 88 ( MyD88 )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we analyzed constitutive monocyte TLR2 expression and evaluated the expression profiles of the proximal downstream adapter molecule myeloid differentiation factor 88 ( MyD88 ) .
	manualset3
85231	1	398292	5	NULL	NULL	0	NULL	Subrenal capsule assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Subrenal capsule assay in normal mice immunosuppressed by cyclosporin A ) .
	manualset3
85232	2	398292	5	NULL	NULL	0	NULL	normal mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Subrenal capsule assay in normal mice immunosuppressed by cyclosporin A ) .
	manualset3
85233	3	398292	5	NULL	NULL	0	NULL	cyclosporin A	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Subrenal capsule assay in normal mice immunosuppressed by cyclosporin A ) .
	manualset3
85234	1	398293	5	NULL	NULL	NULL	NULL	Toll-like receptor-IL-1 receptor signaling components	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we analyzed the Toll-like receptor-IL-1 receptor signaling components involved in the post-transcriptional regulation of IB - with mutated estrogen receptor ( ER ( T2 ) ) fusion proteins .
	manualset3
85235	2	398293	5	NULL	NULL	0	NULL	post-transcriptional regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we analyzed the Toll-like receptor-IL-1 receptor signaling components involved in the post-transcriptional regulation of IB - with mutated estrogen receptor ( ER ( T2 ) ) fusion proteins .
	manualset3
85236	3	398293	5	NULL	NULL	0	NULL	IB	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we analyzed the Toll-like receptor-IL-1 receptor signaling components involved in the post-transcriptional regulation of IB - with mutated estrogen receptor ( ER ( T2 ) ) fusion proteins .
	manualset3
85237	4	398293	5	NULL	NULL	0	NULL	mutated estrogen receptor ( ER ( T2 ) ) fusion proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we analyzed the Toll-like receptor-IL-1 receptor signaling components involved in the post-transcriptional regulation of IB - with mutated estrogen receptor ( ER ( T2 ) ) fusion proteins .
	manualset3
85238	1	398294	5	NULL	NULL	0	NULL	electrophysiological and imaging techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we combine a variety of electrophysiological and imaging techniques and computational modeling to elucidate the mechanisms underlying these spatial and temporal properties of waves in developing mouse retina .
	manualset3
85239	2	398294	5	NULL	NULL	0	NULL	computational modeling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we combine a variety of electrophysiological and imaging techniques and computational modeling to elucidate the mechanisms underlying these spatial and temporal properties of waves in developing mouse retina .
	manualset3
85240	3	398294	5	NULL	NULL	0	NULL	mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we combine a variety of electrophysiological and imaging techniques and computational modeling to elucidate the mechanisms underlying these spatial and temporal properties of waves in developing mouse retina .
	manualset3
85241	4	398294	5	NULL	NULL	0	NULL	spatial and temporal properties	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we combine a variety of electrophysiological and imaging techniques and computational modeling to elucidate the mechanisms underlying these spatial and temporal properties of waves in developing mouse retina .
	manualset3
85242	5	398294	5	NULL	NULL	0	NULL	waves	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we combine a variety of electrophysiological and imaging techniques and computational modeling to elucidate the mechanisms underlying these spatial and temporal properties of waves in developing mouse retina .
	manualset3
85243	6	398294	5	NULL	NULL	0	NULL	developing mouse retina	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we combine a variety of electrophysiological and imaging techniques and computational modeling to elucidate the mechanisms underlying these spatial and temporal properties of waves in developing mouse retina .
	manualset3
85244	1	398295	5	NULL	NULL	0	NULL	nocturnal dynamics	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we compared nocturnal dynamics in plasma concentrations of ACTH/cortisol in 7 patients with Cushing 's disease with those of 7 healthy controls matched in age and sex with the patients .
	manualset3
85246	2	398295	5	NULL	NULL	NULL	NULL	ACTH	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we compared nocturnal dynamics in plasma concentrations of ACTH/cortisol in 7 patients with Cushing 's disease with those of 7 healthy controls matched in age and sex with the patients .
	manualset3
85247	4	398295	5	NULL	NULL	0	NULL	7 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we compared nocturnal dynamics in plasma concentrations of ACTH/cortisol in 7 patients with Cushing 's disease with those of 7 healthy controls matched in age and sex with the patients .
	manualset3
85248	5	398295	5	NULL	NULL	0	NULL	Cushing 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we compared nocturnal dynamics in plasma concentrations of ACTH/cortisol in 7 patients with Cushing 's disease with those of 7 healthy controls matched in age and sex with the patients .
	manualset3
85249	6	398295	5	NULL	NULL	0	NULL	7 healthy controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we compared nocturnal dynamics in plasma concentrations of ACTH/cortisol in 7 patients with Cushing 's disease with those of 7 healthy controls matched in age and sex with the patients .
	manualset3
85250	7	398295	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we compared nocturnal dynamics in plasma concentrations of ACTH/cortisol in 7 patients with Cushing 's disease with those of 7 healthy controls matched in age and sex with the patients .
	manualset3
85437	3	398295	5	NULL	NULL	0	NULL	cortisol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we compared nocturnal dynamics in plasma concentrations of ACTH/cortisol in 7 patients with Cushing 's disease with those of 7 healthy controls matched in age and sex with the patients .
	manualset3
85499	8	398295	5	NULL	NULL	0	NULL	plasma concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we compared nocturnal dynamics in plasma concentrations of ACTH/cortisol in 7 patients with Cushing 's disease with those of 7 healthy controls matched in age and sex with the patients .
	manualset3
85251	1	398296	5	NULL	NULL	0	NULL	postoperative electrophysiological changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we compared the postoperative electrophysiological changes in resting hand tremor after 32 ablations and 12 DBS implantations in patients with severe tremor-dominant idiopathic Parkinson 's disease ( PD ) and essential tremor ( ET ) .
	manualset3
85252	2	398296	5	NULL	NULL	0	NULL	resting hand tremor	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we compared the postoperative electrophysiological changes in resting hand tremor after 32 ablations and 12 DBS implantations in patients with severe tremor-dominant idiopathic Parkinson 's disease ( PD ) and essential tremor ( ET ) .
	manualset3
85253	3	398296	5	NULL	NULL	0	NULL	32 ablations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we compared the postoperative electrophysiological changes in resting hand tremor after 32 ablations and 12 DBS implantations in patients with severe tremor-dominant idiopathic Parkinson 's disease ( PD ) and essential tremor ( ET ) .
	manualset3
85254	4	398296	5	NULL	NULL	0	NULL	12 DBS implantations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we compared the postoperative electrophysiological changes in resting hand tremor after 32 ablations and 12 DBS implantations in patients with severe tremor-dominant idiopathic Parkinson 's disease ( PD ) and essential tremor ( ET ) .
	manualset3
85255	5	398296	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we compared the postoperative electrophysiological changes in resting hand tremor after 32 ablations and 12 DBS implantations in patients with severe tremor-dominant idiopathic Parkinson 's disease ( PD ) and essential tremor ( ET ) .
	manualset3
85256	6	398296	5	NULL	NULL	0	NULL	severe tremor-dominant idiopathic Parkinson 's disease ( PD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we compared the postoperative electrophysiological changes in resting hand tremor after 32 ablations and 12 DBS implantations in patients with severe tremor-dominant idiopathic Parkinson 's disease ( PD ) and essential tremor ( ET ) .
	manualset3
85257	7	398296	5	NULL	NULL	0	NULL	essential tremor ( ET )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we compared the postoperative electrophysiological changes in resting hand tremor after 32 ablations and 12 DBS implantations in patients with severe tremor-dominant idiopathic Parkinson 's disease ( PD ) and essential tremor ( ET ) .
	manualset3
85258	1	398297	5	NULL	NULL	0	NULL	mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we define the mechanism by which ORF45 activates RSKs .
	manualset3
85259	2	398297	5	NULL	NULL	0	NULL	ORF45	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we define the mechanism by which ORF45 activates RSKs .
	manualset3
85260	3	398297	5	NULL	NULL	0	NULL	RSKs	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we define the mechanism by which ORF45 activates RSKs .
	manualset3
85261	1	398298	5	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we defined the role of CXCR5 in the development of mucosal tertiary lymphoid tissue and gastric inflammation in a mouse model of chronic H. pylori infection .
	manualset3
85262	2	398298	5	NULL	NULL	0	NULL	CXCR5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we defined the role of CXCR5 in the development of mucosal tertiary lymphoid tissue and gastric inflammation in a mouse model of chronic H. pylori infection .
	manualset3
85263	3	398298	5	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we defined the role of CXCR5 in the development of mucosal tertiary lymphoid tissue and gastric inflammation in a mouse model of chronic H. pylori infection .
	manualset3
85264	4	398298	5	NULL	NULL	0	NULL	mucosal tertiary lymphoid tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we defined the role of CXCR5 in the development of mucosal tertiary lymphoid tissue and gastric inflammation in a mouse model of chronic H. pylori infection .
	manualset3
85265	5	398298	5	NULL	NULL	0	NULL	gastric inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we defined the role of CXCR5 in the development of mucosal tertiary lymphoid tissue and gastric inflammation in a mouse model of chronic H. pylori infection .
	manualset3
85266	6	398298	5	NULL	NULL	0	NULL	mouse model	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we defined the role of CXCR5 in the development of mucosal tertiary lymphoid tissue and gastric inflammation in a mouse model of chronic H. pylori infection .
	manualset3
85267	7	398298	5	NULL	NULL	0	NULL	chronic H. pylori infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we defined the role of CXCR5 in the development of mucosal tertiary lymphoid tissue and gastric inflammation in a mouse model of chronic H. pylori infection .
	manualset3
85268	1	398299	5	NULL	NULL	0	NULL	Mrc1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we demonstrate that Mrc1 functions constitutively to promote normal replication fork progression .
	manualset3
85269	2	398299	5	NULL	NULL	0	NULL	normal replication fork progression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we demonstrate that Mrc1 functions constitutively to promote normal replication fork progression .
	manualset3
85271	1	398300	5	NULL	NULL	NULL	NULL	vertical and lateral integration	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we demonstrate the vertical and lateral integration of ZnO nanowires into arrays that are capable of producing sufficient power to operate real devices .
	manualset3
85272	2	398300	5	NULL	NULL	0	NULL	ZnO nanowires	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we demonstrate the vertical and lateral integration of ZnO nanowires into arrays that are capable of producing sufficient power to operate real devices .
	manualset3
85273	3	398300	5	NULL	NULL	0	NULL	arrays	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we demonstrate the vertical and lateral integration of ZnO nanowires into arrays that are capable of producing sufficient power to operate real devices .
	manualset3
85274	4	398300	5	NULL	NULL	0	NULL	sufficient power	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we demonstrate the vertical and lateral integration of ZnO nanowires into arrays that are capable of producing sufficient power to operate real devices .
	manualset3
85275	5	398300	5	NULL	NULL	0	NULL	real devices	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we demonstrate the vertical and lateral integration of ZnO nanowires into arrays that are capable of producing sufficient power to operate real devices .
	manualset3
85276	1	398301	5	NULL	NULL	0	NULL	routine nursing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Subtle violence in routine nursing ) .
	manualset3
85277	1	398302	5	NULL	NULL	NULL	NULL	novel and highly conserved paralog of adiponectin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we describe a novel and highly conserved paralog of adiponectin designated as C1q/TNF-related protein ( CTRP ) 9 .
	manualset3
85278	2	398302	5	NULL	NULL	0	NULL	C1q/TNF-related protein ( CTRP ) 9	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we describe a novel and highly conserved paralog of adiponectin designated as C1q/TNF-related protein ( CTRP ) 9 .
	manualset3
85279	1	398303	5	NULL	NULL	0	NULL	novel bacterium	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we describe a novel bacterium , strain TUD-YJ37 ( T ) , which can accumulate polyhydroxybutyrate ( PHB ) to more than 85 % ( w/w ) dry cell weight .
	manualset3
85280	2	398303	5	NULL	NULL	0	NULL	strain TUD-YJ37 ( T )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we describe a novel bacterium , strain TUD-YJ37 ( T ) , which can accumulate polyhydroxybutyrate ( PHB ) to more than 85 % ( w/w ) dry cell weight .
	manualset3
85281	3	398303	5	NULL	NULL	0	NULL	polyhydroxybutyrate ( PHB )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we describe a novel bacterium , strain TUD-YJ37 ( T ) , which can accumulate polyhydroxybutyrate ( PHB ) to more than 85 % ( w/w ) dry cell weight .
	manualset3
85282	4	398303	5	NULL	NULL	0	NULL	85 % ( w/w ) dry cell weight	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we describe a novel bacterium , strain TUD-YJ37 ( T ) , which can accumulate polyhydroxybutyrate ( PHB ) to more than 85 % ( w/w ) dry cell weight .
	manualset3
85283	1	398304	5	NULL	NULL	0	NULL	novel cell biological mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we describe a novel cell biological mechanism that disperses membrane fragments over large distances through the Drosophila imaginal disc epithelium .
	manualset3
85284	2	398304	5	NULL	NULL	0	NULL	membrane fragments	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we describe a novel cell biological mechanism that disperses membrane fragments over large distances through the Drosophila imaginal disc epithelium .
	manualset3
85286	4	398304	5	NULL	NULL	NULL	NULL	Drosophila imaginal disc epithelium	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we describe a novel cell biological mechanism that disperses membrane fragments over large distances through the Drosophila imaginal disc epithelium .
	manualset3
85438	3	398304	5	NULL	NULL	0	NULL	large distances	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we describe a novel cell biological mechanism that disperses membrane fragments over large distances through the Drosophila imaginal disc epithelium .
	manualset3
85287	1	398305	5	NULL	NULL	0	NULL	novel protein molecular weight markers	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we describe novel protein molecular weight markers in which a prestaining procedure is no longer needed .
	manualset3
85288	2	398305	5	NULL	NULL	0	NULL	prestaining procedure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we describe novel protein molecular weight markers in which a prestaining procedure is no longer needed .
	manualset3
85289	1	398306	5	NULL	NULL	0	NULL	 isolation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we describe the isolation of the CMP-Neu5Ac hydroxylase from A. rubens gonads using anion exchange chromatography and chromatography on immobilized cytochrome b ( 5 ) .
	manualset3
85290	2	398306	5	NULL	NULL	0	NULL	CMP-Neu5Ac hydroxylase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we describe the isolation of the CMP-Neu5Ac hydroxylase from A. rubens gonads using anion exchange chromatography and chromatography on immobilized cytochrome b ( 5 ) .
	manualset3
85291	3	398306	5	NULL	NULL	0	NULL	A. rubens gonads	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we describe the isolation of the CMP-Neu5Ac hydroxylase from A. rubens gonads using anion exchange chromatography and chromatography on immobilized cytochrome b ( 5 ) .
	manualset3
85292	4	398306	5	NULL	NULL	0	NULL	anion exchange chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we describe the isolation of the CMP-Neu5Ac hydroxylase from A. rubens gonads using anion exchange chromatography and chromatography on immobilized cytochrome b ( 5 ) .
	manualset3
85293	5	398306	5	NULL	NULL	0	NULL	chromatography on immobilized cytochrome b ( 5 )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we describe the isolation of the CMP-Neu5Ac hydroxylase from A. rubens gonads using anion exchange chromatography and chromatography on immobilized cytochrome b ( 5 ) .
	manualset3
85294	1	398307	5	NULL	NULL	0	NULL	functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we evaluated the functions of the two major signaling pathways , the signal transducers and activators of transcription 1 and 3 ( STAT1/3 ) and the Src-homology tyrosine phosphatase 2 ( SHP2 ) - Ras-ERK , emanating from the common signal transducer , gp130 , in the gastrointestinal tract .
	manualset3
85295	2	398307	5	NULL	NULL	NULL	NULL	major signaling pathways	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we evaluated the functions of the two major signaling pathways , the signal transducers and activators of transcription 1 and 3 ( STAT1/3 ) and the Src-homology tyrosine phosphatase 2 ( SHP2 ) - Ras-ERK , emanating from the common signal transducer , gp130 , in the gastrointestinal tract .
	manualset3
85296	3	398307	5	NULL	NULL	NULL	NULL	signal transducers and activators of transcription 1 and 3 ( STAT1/3 )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we evaluated the functions of the two major signaling pathways , the signal transducers and activators of transcription 1 and 3 ( STAT1/3 ) and the Src-homology tyrosine phosphatase 2 ( SHP2 ) - Ras-ERK , emanating from the common signal transducer , gp130 , in the gastrointestinal tract .
	manualset3
85298	4	398307	5	NULL	NULL	NULL	NULL	Src-homology tyrosine phosphatase 2 ( SHP2 ) - Ras-ERKB signaling pathway	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we evaluated the functions of the two major signaling pathways , the signal transducers and activators of transcription 1 and 3 ( STAT1/3 ) and the Src-homology tyrosine phosphatase 2 ( SHP2 ) - Ras-ERK , emanating from the common signal transducer , gp130 , in the gastrointestinal tract .
	manualset3
85299	5	398307	5	NULL	NULL	NULL	NULL	common signal transducer	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we evaluated the functions of the two major signaling pathways , the signal transducers and activators of transcription 1 and 3 ( STAT1/3 ) and the Src-homology tyrosine phosphatase 2 ( SHP2 ) - Ras-ERK , emanating from the common signal transducer , gp130 , in the gastrointestinal tract .
	manualset3
85300	6	398307	5	NULL	NULL	NULL	NULL	gp130	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we evaluated the functions of the two major signaling pathways , the signal transducers and activators of transcription 1 and 3 ( STAT1/3 ) and the Src-homology tyrosine phosphatase 2 ( SHP2 ) - Ras-ERK , emanating from the common signal transducer , gp130 , in the gastrointestinal tract .
	manualset3
85301	7	398307	5	NULL	NULL	NULL	NULL	gastrointestinal tract	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we evaluated the functions of the two major signaling pathways , the signal transducers and activators of transcription 1 and 3 ( STAT1/3 ) and the Src-homology tyrosine phosphatase 2 ( SHP2 ) - Ras-ERK , emanating from the common signal transducer , gp130 , in the gastrointestinal tract .
	manualset3
85302	1	398308	5	NULL	NULL	0	NULL	cellular distribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we examined cellular distribution of Daxx by sub-cellular fractionation and immunofluorescent localization of endogenous protein , using SH-SY5Y neuroblastoma cell line previously reported to exhibit cytoplasmic translocation of Daxx after oxidative stress and beta-amyloid exposure .
	manualset3
85303	2	398308	5	NULL	NULL	0	NULL	Daxx	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we examined cellular distribution of Daxx by sub-cellular fractionation and immunofluorescent localization of endogenous protein , using SH-SY5Y neuroblastoma cell line previously reported to exhibit cytoplasmic translocation of Daxx after oxidative stress and beta-amyloid exposure .
	manualset3
85304	3	398308	5	NULL	NULL	0	NULL	sub-cellular fractionation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we examined cellular distribution of Daxx by sub-cellular fractionation and immunofluorescent localization of endogenous protein , using SH-SY5Y neuroblastoma cell line previously reported to exhibit cytoplasmic translocation of Daxx after oxidative stress and beta-amyloid exposure .
	manualset3
85305	4	398308	5	NULL	NULL	0	NULL	immunofluorescent localization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we examined cellular distribution of Daxx by sub-cellular fractionation and immunofluorescent localization of endogenous protein , using SH-SY5Y neuroblastoma cell line previously reported to exhibit cytoplasmic translocation of Daxx after oxidative stress and beta-amyloid exposure .
	manualset3
85306	5	398308	5	NULL	NULL	0	NULL	endogenous protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we examined cellular distribution of Daxx by sub-cellular fractionation and immunofluorescent localization of endogenous protein , using SH-SY5Y neuroblastoma cell line previously reported to exhibit cytoplasmic translocation of Daxx after oxidative stress and beta-amyloid exposure .
	manualset3
85307	6	398308	5	NULL	NULL	0	NULL	SH-SY5Y neuroblastoma cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we examined cellular distribution of Daxx by sub-cellular fractionation and immunofluorescent localization of endogenous protein , using SH-SY5Y neuroblastoma cell line previously reported to exhibit cytoplasmic translocation of Daxx after oxidative stress and beta-amyloid exposure .
	manualset3
85308	7	398308	5	NULL	NULL	0	NULL	cytoplasmic translocation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we examined cellular distribution of Daxx by sub-cellular fractionation and immunofluorescent localization of endogenous protein , using SH-SY5Y neuroblastoma cell line previously reported to exhibit cytoplasmic translocation of Daxx after oxidative stress and beta-amyloid exposure .
	manualset3
85309	8	398308	5	NULL	NULL	0	NULL	Daxx	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we examined cellular distribution of Daxx by sub-cellular fractionation and immunofluorescent localization of endogenous protein , using SH-SY5Y neuroblastoma cell line previously reported to exhibit cytoplasmic translocation of Daxx after oxidative stress and beta-amyloid exposure .
	manualset3
85310	9	398308	5	NULL	NULL	0	NULL	oxidative stress	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we examined cellular distribution of Daxx by sub-cellular fractionation and immunofluorescent localization of endogenous protein , using SH-SY5Y neuroblastoma cell line previously reported to exhibit cytoplasmic translocation of Daxx after oxidative stress and beta-amyloid exposure .
	manualset3
85311	10	398308	5	NULL	NULL	0	NULL	beta-amyloid exposure	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we examined cellular distribution of Daxx by sub-cellular fractionation and immunofluorescent localization of endogenous protein , using SH-SY5Y neuroblastoma cell line previously reported to exhibit cytoplasmic translocation of Daxx after oxidative stress and beta-amyloid exposure .
	manualset3
85312	1	398309	5	NULL	NULL	0	NULL	antisense oligonucleotide ( AS ) therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we examined the effects of an antisense oligonucleotide ( AS ) therapy directed against SHIP2 on whole body insulin sensitivity and insulin action in liver and muscle tissue in a dietary rodent model of the metabolic syndrome , the high-fat-fed ( HF ) rat .
	manualset3
85313	2	398309	5	NULL	NULL	0	NULL	SHIP2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we examined the effects of an antisense oligonucleotide ( AS ) therapy directed against SHIP2 on whole body insulin sensitivity and insulin action in liver and muscle tissue in a dietary rodent model of the metabolic syndrome , the high-fat-fed ( HF ) rat .
	manualset3
85314	3	398309	5	NULL	NULL	0	NULL	whole body insulin sensitivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we examined the effects of an antisense oligonucleotide ( AS ) therapy directed against SHIP2 on whole body insulin sensitivity and insulin action in liver and muscle tissue in a dietary rodent model of the metabolic syndrome , the high-fat-fed ( HF ) rat .
	manualset3
85315	4	398309	5	NULL	NULL	0	NULL	insulin action	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we examined the effects of an antisense oligonucleotide ( AS ) therapy directed against SHIP2 on whole body insulin sensitivity and insulin action in liver and muscle tissue in a dietary rodent model of the metabolic syndrome , the high-fat-fed ( HF ) rat .
	manualset3
85316	5	398309	5	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we examined the effects of an antisense oligonucleotide ( AS ) therapy directed against SHIP2 on whole body insulin sensitivity and insulin action in liver and muscle tissue in a dietary rodent model of the metabolic syndrome , the high-fat-fed ( HF ) rat .
	manualset3
85317	6	398309	5	NULL	NULL	0	NULL	muscle tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we examined the effects of an antisense oligonucleotide ( AS ) therapy directed against SHIP2 on whole body insulin sensitivity and insulin action in liver and muscle tissue in a dietary rodent model of the metabolic syndrome , the high-fat-fed ( HF ) rat .
	manualset3
85318	7	398309	5	NULL	NULL	0	NULL	dietary rodent model	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we examined the effects of an antisense oligonucleotide ( AS ) therapy directed against SHIP2 on whole body insulin sensitivity and insulin action in liver and muscle tissue in a dietary rodent model of the metabolic syndrome , the high-fat-fed ( HF ) rat .
	manualset3
85319	8	398309	5	NULL	NULL	0	NULL	metabolic syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we examined the effects of an antisense oligonucleotide ( AS ) therapy directed against SHIP2 on whole body insulin sensitivity and insulin action in liver and muscle tissue in a dietary rodent model of the metabolic syndrome , the high-fat-fed ( HF ) rat .
	manualset3
85320	9	398309	5	NULL	NULL	0	NULL	high-fat-fed ( HF ) rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we examined the effects of an antisense oligonucleotide ( AS ) therapy directed against SHIP2 on whole body insulin sensitivity and insulin action in liver and muscle tissue in a dietary rodent model of the metabolic syndrome , the high-fat-fed ( HF ) rat .
	manualset3
85321	1	398310	5	NULL	NULL	0	NULL	Notch-mediated regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we focus on recent advances in our understanding of Notch-mediated regulation of cardiac development with specific attention to the formation of the cardiac outflow tract .
	manualset3
85322	2	398310	5	NULL	NULL	0	NULL	cardiac development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we focus on recent advances in our understanding of Notch-mediated regulation of cardiac development with specific attention to the formation of the cardiac outflow tract .
	manualset3
85323	3	398310	5	NULL	NULL	0	NULL	specific attention	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we focus on recent advances in our understanding of Notch-mediated regulation of cardiac development with specific attention to the formation of the cardiac outflow tract .
	manualset3
85324	4	398310	5	NULL	NULL	0	NULL	formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we focus on recent advances in our understanding of Notch-mediated regulation of cardiac development with specific attention to the formation of the cardiac outflow tract .
	manualset3
85325	5	398310	5	NULL	NULL	0	NULL	cardiac outflow tract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we focus on recent advances in our understanding of Notch-mediated regulation of cardiac development with specific attention to the formation of the cardiac outflow tract .
	manualset3
85326	1	398311	5	NULL	NULL	0	NULL	Successful treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Successful treatment of cystoid macular edema with etanercept in a patient with rheumatoid arthritis associated panuveitis ) .
	manualset3
85327	2	398311	5	NULL	NULL	0	NULL	cystoid macular edema	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Successful treatment of cystoid macular edema with etanercept in a patient with rheumatoid arthritis associated panuveitis ) .
	manualset3
85328	3	398311	5	NULL	NULL	0	NULL	etanercept	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Successful treatment of cystoid macular edema with etanercept in a patient with rheumatoid arthritis associated panuveitis ) .
	manualset3
85329	4	398311	5	NULL	NULL	0	NULL	patient	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Successful treatment of cystoid macular edema with etanercept in a patient with rheumatoid arthritis associated panuveitis ) .
	manualset3
85330	5	398311	5	NULL	NULL	0	NULL	rheumatoid arthritis associated panuveitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Successful treatment of cystoid macular edema with etanercept in a patient with rheumatoid arthritis associated panuveitis ) .
	manualset3
85331	1	398312	5	NULL	NULL	0	NULL	ADH1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we have examined the involvement of ADH1 and ADH4 in embryonic adrenal function by using transgenic mouse technology and immunohistochemistry .
	manualset3
85332	2	398312	5	NULL	NULL	0	NULL	ADH4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we have examined the involvement of ADH1 and ADH4 in embryonic adrenal function by using transgenic mouse technology and immunohistochemistry .
	manualset3
85333	3	398312	5	NULL	NULL	0	NULL	embryonic adrenal function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we have examined the involvement of ADH1 and ADH4 in embryonic adrenal function by using transgenic mouse technology and immunohistochemistry .
	manualset3
85334	4	398312	5	NULL	NULL	0	NULL	transgenic mouse technology	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we have examined the involvement of ADH1 and ADH4 in embryonic adrenal function by using transgenic mouse technology and immunohistochemistry .
	manualset3
85335	5	398312	5	NULL	NULL	0	NULL	immunohistochemistry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we have examined the involvement of ADH1 and ADH4 in embryonic adrenal function by using transgenic mouse technology and immunohistochemistry .
	manualset3
85336	1	398313	5	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we have further elucidated the role of MMP-13 in tumor invasion by examining its expression in invasive malignant tumors of the female genital tract .
	manualset3
85337	2	398313	5	NULL	NULL	0	NULL	MMP-13	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we have further elucidated the role of MMP-13 in tumor invasion by examining its expression in invasive malignant tumors of the female genital tract .
	manualset3
85338	3	398313	5	NULL	NULL	0	NULL	tumor invasion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we have further elucidated the role of MMP-13 in tumor invasion by examining its expression in invasive malignant tumors of the female genital tract .
	manualset3
85339	4	398313	5	NULL	NULL	0	NULL	expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we have further elucidated the role of MMP-13 in tumor invasion by examining its expression in invasive malignant tumors of the female genital tract .
	manualset3
85340	5	398313	5	NULL	NULL	0	NULL	invasive malignant tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we have further elucidated the role of MMP-13 in tumor invasion by examining its expression in invasive malignant tumors of the female genital tract .
	manualset3
85341	6	398313	5	NULL	NULL	0	NULL	female genital tract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we have further elucidated the role of MMP-13 in tumor invasion by examining its expression in invasive malignant tumors of the female genital tract .
	manualset3
85342	1	398314	5	NULL	NULL	0	NULL	atomic force microsopy ( AFM )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we have used atomic force microsopy ( AFM ) to study the effects of MBP and P2 on lipid bilayers .
	manualset3
85343	2	398314	5	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we have used atomic force microsopy ( AFM ) to study the effects of MBP and P2 on lipid bilayers .
	manualset3
85344	3	398314	5	NULL	NULL	0	NULL	MBP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we have used atomic force microsopy ( AFM ) to study the effects of MBP and P2 on lipid bilayers .
	manualset3
85345	4	398314	5	NULL	NULL	0	NULL	P2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we have used atomic force microsopy ( AFM ) to study the effects of MBP and P2 on lipid bilayers .
	manualset3
85346	5	398314	5	NULL	NULL	NULL	NULL	lipid bilayers	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we have used atomic force microsopy ( AFM ) to study the effects of MBP and P2 on lipid bilayers .
	manualset3
85347	1	398315	5	NULL	NULL	NULL	NULL	RKIP dimer formation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we identify RKIP dimer formation as an important mechanistic feature in the target switch from Raf1 to GRK2 .
	manualset3
85349	2	398315	5	NULL	NULL	NULL	NULL	target switch	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we identify RKIP dimer formation as an important mechanistic feature in the target switch from Raf1 to GRK2 .
	manualset3
85350	3	398315	5	NULL	NULL	NULL	NULL	Raf1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we identify RKIP dimer formation as an important mechanistic feature in the target switch from Raf1 to GRK2 .
	manualset3
85351	4	398315	5	NULL	NULL	NULL	NULL	GRK2	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we identify RKIP dimer formation as an important mechanistic feature in the target switch from Raf1 to GRK2 .
	manualset3
85352	1	398316	5	NULL	NULL	0	NULL	nakiterpiosin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we identify nakiterpiosin as a novel antimitotic drug that targets microtubules .
	manualset3
85353	2	398316	5	NULL	NULL	0	NULL	novel antimitotic drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we identify nakiterpiosin as a novel antimitotic drug that targets microtubules .
	manualset3
85354	3	398316	5	NULL	NULL	0	NULL	microtubules	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we identify nakiterpiosin as a novel antimitotic drug that targets microtubules .
	manualset3
85355	1	398317	5	NULL	NULL	0	NULL	 interactive computer application	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we introduce an interactive computer application with a graphical interface , for the purpose of educating students about DP .
	manualset3
85356	2	398317	5	NULL	NULL	NULL	NULL	graphical interface	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we introduce an interactive computer application with a graphical interface , for the purpose of educating students about DP .
	manualset3
85357	3	398317	5	NULL	NULL	0	NULL	students	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we introduce an interactive computer application with a graphical interface , for the purpose of educating students about DP .
	manualset3
85358	4	398317	5	NULL	NULL	0	NULL	DP	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we introduce an interactive computer application with a graphical interface , for the purpose of educating students about DP .
	manualset3
85359	1	398318	5	NULL	NULL	0	NULL	investigation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( An investigation on the prevalence of internet addiction disorder in middle school students of Hunan province ) .
	manualset3
85360	2	398318	5	NULL	NULL	0	NULL	internet addiction disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( An investigation on the prevalence of internet addiction disorder in middle school students of Hunan province ) .
	manualset3
85361	3	398318	5	NULL	NULL	0	NULL	middle school students	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( An investigation on the prevalence of internet addiction disorder in middle school students of Hunan province ) .
	manualset3
85362	4	398318	5	NULL	NULL	0	NULL	Hunan province	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( An investigation on the prevalence of internet addiction disorder in middle school students of Hunan province ) .
	manualset3
85363	1	398319	5	NULL	NULL	0	NULL	Suppression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Suppression of pituitary-adrenal axis by triamcinolone acetonide in asthmatics ) .
	manualset3
85364	2	398319	5	NULL	NULL	0	NULL	pituitary-adrenal axis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Suppression of pituitary-adrenal axis by triamcinolone acetonide in asthmatics ) .
	manualset3
85365	3	398319	5	NULL	NULL	0	NULL	triamcinolone acetonide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Suppression of pituitary-adrenal axis by triamcinolone acetonide in asthmatics ) .
	manualset3
85366	4	398319	5	NULL	NULL	0	NULL	asthmatics	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Suppression of pituitary-adrenal axis by triamcinolone acetonide in asthmatics ) .
	manualset3
85367	1	398320	5	NULL	NULL	0	NULL	activating role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we investigated the activating role of the second and third extracellular loop of the human adenosine A1 receptor .
	manualset3
85368	2	398320	5	NULL	NULL	0	NULL	second and third extracellular loop	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we investigated the activating role of the second and third extracellular loop of the human adenosine A1 receptor .
	manualset3
85369	3	398320	5	NULL	NULL	0	NULL	human adenosine A1 receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we investigated the activating role of the second and third extracellular loop of the human adenosine A1 receptor .
	manualset3
85370	1	398321	5	NULL	NULL	0	NULL	ecologically relevant levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we investigated the effects of ecologically relevant levels of UVR on the transmission of the intertidal trematode Maritrema novaezealandensis from its first intermediate snail host ( Zeacumantus subcarinatus ) to its second intermediate amphipod host ( Paracalliope novizealandiae ) .
	manualset3
85371	2	398321	5	NULL	NULL	0	NULL	UVR	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we investigated the effects of ecologically relevant levels of UVR on the transmission of the intertidal trematode Maritrema novaezealandensis from its first intermediate snail host ( Zeacumantus subcarinatus ) to its second intermediate amphipod host ( Paracalliope novizealandiae ) .
	manualset3
85372	3	398321	5	NULL	NULL	0	NULL	transmission	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we investigated the effects of ecologically relevant levels of UVR on the transmission of the intertidal trematode Maritrema novaezealandensis from its first intermediate snail host ( Zeacumantus subcarinatus ) to its second intermediate amphipod host ( Paracalliope novizealandiae ) .
	manualset3
85373	4	398321	5	NULL	NULL	0	NULL	 intertidal trematode Maritrema novaezealandensis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we investigated the effects of ecologically relevant levels of UVR on the transmission of the intertidal trematode Maritrema novaezealandensis from its first intermediate snail host ( Zeacumantus subcarinatus ) to its second intermediate amphipod host ( Paracalliope novizealandiae ) .
	manualset3
85374	5	398321	5	NULL	NULL	NULL	NULL	 Zeacumantus subcarinatus	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we investigated the effects of ecologically relevant levels of UVR on the transmission of the intertidal trematode Maritrema novaezealandensis from its first intermediate snail host ( Zeacumantus subcarinatus ) to its second intermediate amphipod host ( Paracalliope novizealandiae ) .
	manualset3
85375	6	398321	5	NULL	NULL	NULL	NULL	Paracalliope novizealandiae	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we investigated the effects of ecologically relevant levels of UVR on the transmission of the intertidal trematode Maritrema novaezealandensis from its first intermediate snail host ( Zeacumantus subcarinatus ) to its second intermediate amphipod host ( Paracalliope novizealandiae ) .
	manualset3
85377	1	398322	5	NULL	NULL	NULL	NULL	extracts of anterior and posterior cockroach midguts	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we partially purified extracts of anterior and posterior cockroach midguts , using HPLC coupled with radioimmunoassay , and found , among multiple FMRFamide-like immunoreactive fractions , one fraction co-eluting with LMS in both regions .
	manualset3
85378	2	398322	5	NULL	NULL	NULL	NULL	HPLC coupled with radioimmunoassay	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we partially purified extracts of anterior and posterior cockroach midguts , using HPLC coupled with radioimmunoassay , and found , among multiple FMRFamide-like immunoreactive fractions , one fraction co-eluting with LMS in both regions .
	manualset3
85379	3	398322	5	NULL	NULL	NULL	NULL	FMRFamide-like immunoreactive fractions	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we partially purified extracts of anterior and posterior cockroach midguts , using HPLC coupled with radioimmunoassay , and found , among multiple FMRFamide-like immunoreactive fractions , one fraction co-eluting with LMS in both regions .
	manualset3
85380	4	398322	5	NULL	NULL	NULL	NULL	one fraction	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we partially purified extracts of anterior and posterior cockroach midguts , using HPLC coupled with radioimmunoassay , and found , among multiple FMRFamide-like immunoreactive fractions , one fraction co-eluting with LMS in both regions .
	manualset3
85381	1	398323	5	NULL	NULL	0	NULL	visualized current-clamp recordings	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we performed visualized current-clamp recordings to determine the effects of repeated cocaine administration on the membrane excitability of mPFC pyramidal neurons in rat brain slices .
	manualset3
85382	2	398323	5	NULL	NULL	0	NULL	repeated cocaine administration	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we performed visualized current-clamp recordings to determine the effects of repeated cocaine administration on the membrane excitability of mPFC pyramidal neurons in rat brain slices .
	manualset3
85383	3	398323	5	NULL	NULL	0	NULL	membrane excitability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we performed visualized current-clamp recordings to determine the effects of repeated cocaine administration on the membrane excitability of mPFC pyramidal neurons in rat brain slices .
	manualset3
85384	4	398323	5	NULL	NULL	0	NULL	mPFC pyramidal neurons	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we performed visualized current-clamp recordings to determine the effects of repeated cocaine administration on the membrane excitability of mPFC pyramidal neurons in rat brain slices .
	manualset3
85385	5	398323	5	NULL	NULL	0	NULL	rat brain slices	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we performed visualized current-clamp recordings to determine the effects of repeated cocaine administration on the membrane excitability of mPFC pyramidal neurons in rat brain slices .
	manualset3
85386	1	398324	5	NULL	NULL	0	NULL	direct proteomic approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we present a direct proteomic approach , used to study the degree of iodination of mouse Tg without any preliminary purification .
	manualset3
85387	2	398324	5	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we present a direct proteomic approach , used to study the degree of iodination of mouse Tg without any preliminary purification .
	manualset3
85388	3	398324	5	NULL	NULL	0	NULL	degree of iodination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we present a direct proteomic approach , used to study the degree of iodination of mouse Tg without any preliminary purification .
	manualset3
85389	4	398324	5	NULL	NULL	0	NULL	mouse Tg	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we present a direct proteomic approach , used to study the degree of iodination of mouse Tg without any preliminary purification .
	manualset3
85390	5	398324	5	NULL	NULL	0	NULL	preliminary purification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we present a direct proteomic approach , used to study the degree of iodination of mouse Tg without any preliminary purification .
	manualset3
85391	1	398325	5	NULL	NULL	0	NULL	unusual case	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we present an unusual case of unilateral leg calciphylaxis in the setting of relative chronic arterial insufficiency of the affected extremity secondary to steal syndrome .
	manualset3
85392	2	398325	5	NULL	NULL	0	NULL	unilateral leg calciphylaxis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we present an unusual case of unilateral leg calciphylaxis in the setting of relative chronic arterial insufficiency of the affected extremity secondary to steal syndrome .
	manualset3
85393	3	398325	5	NULL	NULL	0	NULL	relative chronic arterial insufficiency	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we present an unusual case of unilateral leg calciphylaxis in the setting of relative chronic arterial insufficiency of the affected extremity secondary to steal syndrome .
	manualset3
85394	4	398325	5	NULL	NULL	0	NULL	steal syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we present an unusual case of unilateral leg calciphylaxis in the setting of relative chronic arterial insufficiency of the affected extremity secondary to steal syndrome .
	manualset3
85395	1	398326	5	NULL	NULL	0	NULL	critical role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we present evidence identifying a critical role for Hsp90 in TGFbeta signaling .
	manualset3
85396	2	398326	5	NULL	NULL	0	NULL	Hsp90	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we present evidence identifying a critical role for Hsp90 in TGFbeta signaling .
	manualset3
85397	3	398326	5	NULL	NULL	0	NULL	TGFbeta signaling	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we present evidence identifying a critical role for Hsp90 in TGFbeta signaling .
	manualset3
85398	1	398327	5	NULL	NULL	NULL	NULL	simple DNA gate architecture	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we propose a simple DNA gate architecture that appears suitable for practical synthesis of large-scale circuits involving possibly thousands of gates .
	manualset3
85399	2	398327	5	NULL	NULL	0	NULL	practical synthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we propose a simple DNA gate architecture that appears suitable for practical synthesis of large-scale circuits involving possibly thousands of gates .
	manualset3
85402	1	398328	5	NULL	NULL	0	NULL	case	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report a case of spondylitis due to brucella in an elderly male .
	manualset3
85403	2	398328	5	NULL	NULL	0	NULL	spondylitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report a case of spondylitis due to brucella in an elderly male .
	manualset3
85404	3	398328	5	NULL	NULL	0	NULL	brucella	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report a case of spondylitis due to brucella in an elderly male .
	manualset3
85405	4	398328	5	NULL	NULL	0	NULL	elderly male	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report a case of spondylitis due to brucella in an elderly male .
	manualset3
85406	1	398329	5	NULL	NULL	0	NULL	miR expression profile	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report changes in miR expression profile in hepatocellular carcinomas ( HCCs ) developed in male Fisher rats-fed folic acid , methionine , and choline-deficient ( FMD ) diet .
	manualset3
85407	2	398329	5	NULL	NULL	0	NULL	hepatocellular carcinomas ( HCCs )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report changes in miR expression profile in hepatocellular carcinomas ( HCCs ) developed in male Fisher rats-fed folic acid , methionine , and choline-deficient ( FMD ) diet .
	manualset3
85408	3	398329	5	NULL	NULL	0	NULL	male Fisher rats-fed folic acid , methionine , and choline-deficient ( FMD ) diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report changes in miR expression profile in hepatocellular carcinomas ( HCCs ) developed in male Fisher rats-fed folic acid , methionine , and choline-deficient ( FMD ) diet .
	manualset3
85409	1	398330	5	NULL	NULL	0	NULL	Surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Surgery on the smoking habits of juveniles ) .
	manualset3
85410	2	398330	5	NULL	NULL	0	NULL	smoking habits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Surgery on the smoking habits of juveniles ) .
	manualset3
85411	3	398330	5	NULL	NULL	0	NULL	juveniles	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Surgery on the smoking habits of juveniles ) .
	manualset3
85439	1	398331	5	NULL	NULL	0	NULL	GATA-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that GATA-2 is expressed in a substantial proportion of prostate cancers and that high expression of GATA-2 is associated with biochemical recurrence and distant metastatic progression in a validation set of 203 cancers .
	manualset3
85440	2	398331	5	NULL	NULL	0	NULL	prostate cancers	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that GATA-2 is expressed in a substantial proportion of prostate cancers and that high expression of GATA-2 is associated with biochemical recurrence and distant metastatic progression in a validation set of 203 cancers .
	manualset3
85441	3	398331	5	NULL	NULL	0	NULL	high expression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that GATA-2 is expressed in a substantial proportion of prostate cancers and that high expression of GATA-2 is associated with biochemical recurrence and distant metastatic progression in a validation set of 203 cancers .
	manualset3
85442	4	398331	5	NULL	NULL	0	NULL	GATA-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that GATA-2 is expressed in a substantial proportion of prostate cancers and that high expression of GATA-2 is associated with biochemical recurrence and distant metastatic progression in a validation set of 203 cancers .
	manualset3
85443	5	398331	5	NULL	NULL	0	NULL	biochemical recurrence and distant metastatic progression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that GATA-2 is expressed in a substantial proportion of prostate cancers and that high expression of GATA-2 is associated with biochemical recurrence and distant metastatic progression in a validation set of 203 cancers .
	manualset3
85444	6	398331	5	NULL	NULL	NULL	NULL	validation set	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we report that GATA-2 is expressed in a substantial proportion of prostate cancers and that high expression of GATA-2 is associated with biochemical recurrence and distant metastatic progression in a validation set of 203 cancers .
	manualset3
86455	7	398331	5	NULL	NULL	0	NULL	203 cancers	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that GATA-2 is expressed in a substantial proportion of prostate cancers and that high expression of GATA-2 is associated with biochemical recurrence and distant metastatic progression in a validation set of 203 cancers .
	manualset3
85445	1	398332	5	NULL	NULL	0	NULL	HBXIP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that HBXIP contributes to protecting breast cancer cells from CDC by upregulating membrane-bound complement regulatory protein ( mCRPs ) , including CD46 , CD55 and CD59 .
	manualset3
85446	2	398332	5	NULL	NULL	0	NULL	breast cancer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that HBXIP contributes to protecting breast cancer cells from CDC by upregulating membrane-bound complement regulatory protein ( mCRPs ) , including CD46 , CD55 and CD59 .
	manualset3
85447	3	398332	5	NULL	NULL	0	NULL	CDC	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that HBXIP contributes to protecting breast cancer cells from CDC by upregulating membrane-bound complement regulatory protein ( mCRPs ) , including CD46 , CD55 and CD59 .
	manualset3
85448	4	398332	5	NULL	NULL	0	NULL	membrane-bound complement regulatory protein ( mCRPs )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that HBXIP contributes to protecting breast cancer cells from CDC by upregulating membrane-bound complement regulatory protein ( mCRPs ) , including CD46 , CD55 and CD59 .
	manualset3
85449	5	398332	5	NULL	NULL	0	NULL	CD46	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that HBXIP contributes to protecting breast cancer cells from CDC by upregulating membrane-bound complement regulatory protein ( mCRPs ) , including CD46 , CD55 and CD59 .
	manualset3
85450	6	398332	5	NULL	NULL	0	NULL	CD55	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that HBXIP contributes to protecting breast cancer cells from CDC by upregulating membrane-bound complement regulatory protein ( mCRPs ) , including CD46 , CD55 and CD59 .
	manualset3
85451	7	398332	5	NULL	NULL	0	NULL	CD59	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that HBXIP contributes to protecting breast cancer cells from CDC by upregulating membrane-bound complement regulatory protein ( mCRPs ) , including CD46 , CD55 and CD59 .
	manualset3
85452	1	398333	5	NULL	NULL	0	NULL	Shank proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that Shank proteins also bind to Homer .
	manualset3
85453	2	398333	5	NULL	NULL	0	NULL	Homer	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that Shank proteins also bind to Homer .
	manualset3
85454	1	398334	5	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that activation of P2Y ( 2 ) receptors by extracellular UTP inhibits the IGF-I-induced p110alpha-PI3K activation .
	manualset3
85455	2	398334	5	NULL	NULL	0	NULL	P2Y ( 2 ) receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that activation of P2Y ( 2 ) receptors by extracellular UTP inhibits the IGF-I-induced p110alpha-PI3K activation .
	manualset3
85456	3	398334	5	NULL	NULL	0	NULL	extracellular UTP	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that activation of P2Y ( 2 ) receptors by extracellular UTP inhibits the IGF-I-induced p110alpha-PI3K activation .
	manualset3
85457	4	398334	5	NULL	NULL	0	NULL	IGF-I-induced p110alpha-PI3K activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that activation of P2Y ( 2 ) receptors by extracellular UTP inhibits the IGF-I-induced p110alpha-PI3K activation .
	manualset3
85458	1	398335	5	NULL	NULL	0	NULL	glucose levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that glucose levels are significantly lower in bulk tumor specimens than those in normal tissues of the same tissue origins .
	manualset3
85459	2	398335	5	NULL	NULL	0	NULL	bulk tumor specimens	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that glucose levels are significantly lower in bulk tumor specimens than those in normal tissues of the same tissue origins .
	manualset3
85460	3	398335	5	NULL	NULL	0	NULL	normal tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that glucose levels are significantly lower in bulk tumor specimens than those in normal tissues of the same tissue origins .
	manualset3
85461	4	398335	5	NULL	NULL	0	NULL	same tissue origins	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that glucose levels are significantly lower in bulk tumor specimens than those in normal tissues of the same tissue origins .
	manualset3
85462	1	398336	5	NULL	NULL	0	NULL	iPLA ( 2 ) expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that iPLA ( 2 ) expression increases in the vascular tunica media upon carotid artery ligation and that neointima formation is suppressed by genetic deletion of iPLA ( 2 ) or by inhibiting its activity or expression via perivascular delivery of bromoenol lactone or of antisense oligonucleotides , respectively .
	manualset3
85463	2	398336	5	NULL	NULL	0	NULL	vascular tunica media	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that iPLA ( 2 ) expression increases in the vascular tunica media upon carotid artery ligation and that neointima formation is suppressed by genetic deletion of iPLA ( 2 ) or by inhibiting its activity or expression via perivascular delivery of bromoenol lactone or of antisense oligonucleotides , respectively .
	manualset3
85464	3	398336	5	NULL	NULL	0	NULL	carotid artery ligation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that iPLA ( 2 ) expression increases in the vascular tunica media upon carotid artery ligation and that neointima formation is suppressed by genetic deletion of iPLA ( 2 ) or by inhibiting its activity or expression via perivascular delivery of bromoenol lactone or of antisense oligonucleotides , respectively .
	manualset3
85465	4	398336	5	NULL	NULL	0	NULL	neointima formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that iPLA ( 2 ) expression increases in the vascular tunica media upon carotid artery ligation and that neointima formation is suppressed by genetic deletion of iPLA ( 2 ) or by inhibiting its activity or expression via perivascular delivery of bromoenol lactone or of antisense oligonucleotides , respectively .
	manualset3
85466	5	398336	5	NULL	NULL	NULL	NULL	genetic deletion	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we report that iPLA ( 2 ) expression increases in the vascular tunica media upon carotid artery ligation and that neointima formation is suppressed by genetic deletion of iPLA ( 2 ) or by inhibiting its activity or expression via perivascular delivery of bromoenol lactone or of antisense oligonucleotides , respectively .
	manualset3
85467	7	398336	5	NULL	NULL	NULL	NULL	activity or expression via perivascular delivery	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we report that iPLA ( 2 ) expression increases in the vascular tunica media upon carotid artery ligation and that neointima formation is suppressed by genetic deletion of iPLA ( 2 ) or by inhibiting its activity or expression via perivascular delivery of bromoenol lactone or of antisense oligonucleotides , respectively .
	manualset3
85468	8	398336	5	NULL	NULL	NULL	NULL	bromoenol lactone	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we report that iPLA ( 2 ) expression increases in the vascular tunica media upon carotid artery ligation and that neointima formation is suppressed by genetic deletion of iPLA ( 2 ) or by inhibiting its activity or expression via perivascular delivery of bromoenol lactone or of antisense oligonucleotides , respectively .
	manualset3
85469	9	398336	5	NULL	NULL	NULL	NULL	antisense oligonucleotides	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we report that iPLA ( 2 ) expression increases in the vascular tunica media upon carotid artery ligation and that neointima formation is suppressed by genetic deletion of iPLA ( 2 ) or by inhibiting its activity or expression via perivascular delivery of bromoenol lactone or of antisense oligonucleotides , respectively .
	manualset3
86456	6	398336	5	NULL	NULL	0	NULL	iPLA ( 2 )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that iPLA ( 2 ) expression increases in the vascular tunica media upon carotid artery ligation and that neointima formation is suppressed by genetic deletion of iPLA ( 2 ) or by inhibiting its activity or expression via perivascular delivery of bromoenol lactone or of antisense oligonucleotides , respectively .
	manualset3
85470	1	398337	5	NULL	NULL	0	NULL	maternally contributed fat facets ( faf ; a homolog of USP9X/FAM )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that maternally contributed fat facets ( faf ; a homolog of USP9X/FAM ) is essential for proper interpretation of the zygotic Decapentaplegic ( Dpp ) morphogen gradient that patterns the embryonic dorsal-ventral axis .
	manualset3
85471	2	398337	5	NULL	NULL	0	NULL	proper interpretation	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that maternally contributed fat facets ( faf ; a homolog of USP9X/FAM ) is essential for proper interpretation of the zygotic Decapentaplegic ( Dpp ) morphogen gradient that patterns the embryonic dorsal-ventral axis .
	manualset3
85479	3	398337	5	NULL	NULL	0	NULL	zygotic Decapentaplegic ( Dpp ) morphogen gradient	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that maternally contributed fat facets ( faf ; a homolog of USP9X/FAM ) is essential for proper interpretation of the zygotic Decapentaplegic ( Dpp ) morphogen gradient that patterns the embryonic dorsal-ventral axis .
	manualset3
85480	4	398337	5	NULL	NULL	0	NULL	embryonic dorsal-ventral axis	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that maternally contributed fat facets ( faf ; a homolog of USP9X/FAM ) is essential for proper interpretation of the zygotic Decapentaplegic ( Dpp ) morphogen gradient that patterns the embryonic dorsal-ventral axis .
	manualset3
85481	1	398338	5	NULL	NULL	0	NULL	nuclear import	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that the nuclear import of the various CtBP proteins and splice isoforms is differentially regulated .
	manualset3
85482	2	398338	5	NULL	NULL	0	NULL	CtBP proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that the nuclear import of the various CtBP proteins and splice isoforms is differentially regulated .
	manualset3
85483	3	398338	5	NULL	NULL	0	NULL	splice isoforms	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that the nuclear import of the various CtBP proteins and splice isoforms is differentially regulated .
	manualset3
85484	1	398339	5	NULL	NULL	0	NULL	type 1 T helper cell-like effector cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that type 1 T helper cell-like effector cells that arose in tumor-bearing hosts progressively expressed programmed death 1 during tumor growth .
	manualset3
85485	2	398339	5	NULL	NULL	0	NULL	tumor-bearing hosts	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that type 1 T helper cell-like effector cells that arose in tumor-bearing hosts progressively expressed programmed death 1 during tumor growth .
	manualset3
85486	3	398339	5	NULL	NULL	0	NULL	programmed death 1	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that type 1 T helper cell-like effector cells that arose in tumor-bearing hosts progressively expressed programmed death 1 during tumor growth .
	manualset3
85487	4	398339	5	NULL	NULL	0	NULL	tumor growth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that type 1 T helper cell-like effector cells that arose in tumor-bearing hosts progressively expressed programmed death 1 during tumor growth .
	manualset3
85488	1	398340	5	NULL	NULL	0	NULL	metallo -- lactamase HVO_2763	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report the characterisation of this metallo -- lactamase HVO_2763 in the halophilic archaeon Haloferax volcanii .
	manualset3
85489	2	398340	5	NULL	NULL	0	NULL	halophilic archaeon Haloferax volcanii	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report the characterisation of this metallo -- lactamase HVO_2763 in the halophilic archaeon Haloferax volcanii .
	manualset3
85490	1	398341	5	NULL	NULL	0	NULL	Surgical aspects	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Surgical aspects of chronic kidney failure and transplantation .
	manualset3
85491	2	398341	5	NULL	NULL	0	NULL	chronic kidney failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Surgical aspects of chronic kidney failure and transplantation .
	manualset3
85492	3	398341	5	NULL	NULL	0	NULL	transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Surgical aspects of chronic kidney failure and transplantation .
	manualset3
85493	2	398342	5	NULL	NULL	NULL	NULL	novel TCS	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we report the characterization of this novel TCS , designated as RapA1/A2 ( regulation of both actinorhodin and a type I polyketide ) , using genetic and proteomic approaches .
	manualset3
85494	3	398342	5	NULL	NULL	0	NULL	RapA1/A2 ( regulation of both actinorhodin and a type I polyketide )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report the characterization of this novel TCS , designated as RapA1/A2 ( regulation of both actinorhodin and a type I polyketide ) , using genetic and proteomic approaches .
	manualset3
85495	1	398342	5	NULL	NULL	0	NULL	characterization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report the characterization of this novel TCS , designated as RapA1/A2 ( regulation of both actinorhodin and a type I polyketide ) , using genetic and proteomic approaches .
	manualset3
85496	4	398342	5	NULL	NULL	0	NULL	genetic and proteomic approaches	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report the characterization of this novel TCS , designated as RapA1/A2 ( regulation of both actinorhodin and a type I polyketide ) , using genetic and proteomic approaches .
	manualset3
85497	1	398343	5	NULL	NULL	0	NULL	first study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report the first study of synonymous and nonsynonymous substitution rates on plant sex chromosomes .
	manualset3
85509	2	398343	5	NULL	NULL	NULL	NULL	synonymous and nonsynonymous substitution rates	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we report the first study of synonymous and nonsynonymous substitution rates on plant sex chromosomes .
	manualset3
85510	3	398343	5	NULL	NULL	0	NULL	plant sex chromosomes	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report the first study of synonymous and nonsynonymous substitution rates on plant sex chromosomes .
	manualset3
85512	1	398344	5	NULL	NULL	0	NULL	identification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report the identification of a new tomato XET gene , LeXET2 , that shows a different spatial expression and diametrically opposite pattern of auxin regulation from LeEXT .
	manualset3
85513	2	398344	5	NULL	NULL	0	NULL	new tomato XET gene , LeXET2	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report the identification of a new tomato XET gene , LeXET2 , that shows a different spatial expression and diametrically opposite pattern of auxin regulation from LeEXT .
	manualset3
85515	3	398344	5	NULL	NULL	0	NULL	different spatial expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report the identification of a new tomato XET gene , LeXET2 , that shows a different spatial expression and diametrically opposite pattern of auxin regulation from LeEXT .
	manualset3
85516	4	398344	5	NULL	NULL	0	NULL	diametrically opposite pattern of auxin regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report the identification of a new tomato XET gene , LeXET2 , that shows a different spatial expression and diametrically opposite pattern of auxin regulation from LeEXT .
	manualset3
85517	5	398344	5	NULL	NULL	0	NULL	LeEXT	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report the identification of a new tomato XET gene , LeXET2 , that shows a different spatial expression and diametrically opposite pattern of auxin regulation from LeEXT .
	manualset3
85518	1	398345	5	NULL	NULL	0	NULL	behavioural and neuroimaging studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we review recent behavioural and neuroimaging studies on adolescent development of the self-concept .
	manualset3
85519	2	398345	5	NULL	NULL	0	NULL	adolescent development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we review recent behavioural and neuroimaging studies on adolescent development of the self-concept .
	manualset3
85520	3	398345	5	NULL	NULL	0	NULL	self-concept	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we review recent behavioural and neuroimaging studies on adolescent development of the self-concept .
	manualset3
85521	1	398346	5	NULL	NULL	0	NULL	molecular pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we review recent insights into the molecular pathways regulating trophoblast lineage segregation , stem cell maintenance , and subtype differentiation .
	manualset3
85522	2	398346	5	NULL	NULL	0	NULL	trophoblast lineage segregation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we review recent insights into the molecular pathways regulating trophoblast lineage segregation , stem cell maintenance , and subtype differentiation .
	manualset3
85523	3	398346	5	NULL	NULL	0	NULL	stem cell maintenance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we review recent insights into the molecular pathways regulating trophoblast lineage segregation , stem cell maintenance , and subtype differentiation .
	manualset3
85524	4	398346	5	NULL	NULL	0	NULL	subtype differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we review recent insights into the molecular pathways regulating trophoblast lineage segregation , stem cell maintenance , and subtype differentiation .
	manualset3
85533	3	398347	5	NULL	NULL	NULL	NULL	cytokines	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we review the key factors that generate such diversity , as well as the cytokines and transcription factors that are differentially expressed in pathogenic and nonpathogenic Th17 cells .
	manualset3
85534	4	398347	5	NULL	NULL	NULL	NULL	transcription factors	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we review the key factors that generate such diversity , as well as the cytokines and transcription factors that are differentially expressed in pathogenic and nonpathogenic Th17 cells .
	manualset3
85535	5	398347	5	NULL	NULL	NULL	NULL	pathogenic and nonpathogenic Th17 cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we review the key factors that generate such diversity , as well as the cytokines and transcription factors that are differentially expressed in pathogenic and nonpathogenic Th17 cells .
	manualset3
86460	1	398347	5	NULL	NULL	NULL	NULL	key factors	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we review the key factors that generate such diversity , as well as the cytokines and transcription factors that are differentially expressed in pathogenic and nonpathogenic Th17 cells .
	manualset3
86461	2	398347	5	NULL	NULL	NULL	NULL	diversity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we review the key factors that generate such diversity , as well as the cytokines and transcription factors that are differentially expressed in pathogenic and nonpathogenic Th17 cells .
	manualset3
85537	1	398348	5	NULL	NULL	NULL	NULL	medicinal and industrial applications	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we review the medicinal and industrial applications of saffron .
	manualset3
85576	2	398348	5	NULL	NULL	NULL	NULL	saffron	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we review the medicinal and industrial applications of saffron .
	manualset3
85577	1	398349	5	NULL	NULL	NULL	NULL	 novel biodegradable thermosensitive implant	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we show a novel biodegradable thermosensitive implant composed of poly ( ethylene glycol ) monomethyl ether ( mPEG ) and poly ( lactic-co-glycolic acid ) ( PLGA ) copolymer as a sol-gel drug delivery system for treating bone infection .
	manualset3
85578	2	398349	5	NULL	NULL	0	NULL	poly ( ethylene glycol ) monomethyl ether ( mPEG )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show a novel biodegradable thermosensitive implant composed of poly ( ethylene glycol ) monomethyl ether ( mPEG ) and poly ( lactic-co-glycolic acid ) ( PLGA ) copolymer as a sol-gel drug delivery system for treating bone infection .
	manualset3
85579	3	398349	5	NULL	NULL	0	NULL	poly ( lactic-co-glycolic acid ) ( PLGA ) copolymer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show a novel biodegradable thermosensitive implant composed of poly ( ethylene glycol ) monomethyl ether ( mPEG ) and poly ( lactic-co-glycolic acid ) ( PLGA ) copolymer as a sol-gel drug delivery system for treating bone infection .
	manualset3
85580	4	398349	5	NULL	NULL	0	NULL	sol-gel drug delivery system	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show a novel biodegradable thermosensitive implant composed of poly ( ethylene glycol ) monomethyl ether ( mPEG ) and poly ( lactic-co-glycolic acid ) ( PLGA ) copolymer as a sol-gel drug delivery system for treating bone infection .
	manualset3
85581	5	398349	5	NULL	NULL	0	NULL	bone infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show a novel biodegradable thermosensitive implant composed of poly ( ethylene glycol ) monomethyl ether ( mPEG ) and poly ( lactic-co-glycolic acid ) ( PLGA ) copolymer as a sol-gel drug delivery system for treating bone infection .
	manualset3
85582	1	398350	5	NULL	NULL	0	NULL	immunofluorescence experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show by immunofluorescence experiments , in cells exposed to ROS , the involvement of MutY glycosylase homolog ( MUTYH ) and DNA pol lambda in the repair of A : 8 - oxo-G mispairs .
	manualset3
85583	2	398350	5	NULL	NULL	0	NULL	cells exposed to ROS	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show by immunofluorescence experiments , in cells exposed to ROS , the involvement of MutY glycosylase homolog ( MUTYH ) and DNA pol lambda in the repair of A : 8 - oxo-G mispairs .
	manualset3
85584	3	398350	5	NULL	NULL	0	NULL	MutY glycosylase homolog ( MUTYH )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show by immunofluorescence experiments , in cells exposed to ROS , the involvement of MutY glycosylase homolog ( MUTYH ) and DNA pol lambda in the repair of A : 8 - oxo-G mispairs .
	manualset3
85585	4	398350	5	NULL	NULL	0	NULL	DNA pol lambda	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show by immunofluorescence experiments , in cells exposed to ROS , the involvement of MutY glycosylase homolog ( MUTYH ) and DNA pol lambda in the repair of A : 8 - oxo-G mispairs .
	manualset3
85586	5	398350	5	NULL	NULL	0	NULL	repair	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show by immunofluorescence experiments , in cells exposed to ROS , the involvement of MutY glycosylase homolog ( MUTYH ) and DNA pol lambda in the repair of A : 8 - oxo-G mispairs .
	manualset3
85587	6	398350	5	NULL	NULL	NULL	NULL	A : 8 - oxo-G mispairs	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we show by immunofluorescence experiments , in cells exposed to ROS , the involvement of MutY glycosylase homolog ( MUTYH ) and DNA pol lambda in the repair of A : 8 - oxo-G mispairs .
	manualset3
85588	1	398351	5	NULL	NULL	0	NULL	Surgical closure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Surgical closure of perforations of the palate ( suction perforations ) ) .
	manualset3
85589	2	398351	5	NULL	NULL	0	NULL	perforations of the palate ( suction perforations )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Surgical closure of perforations of the palate ( suction perforations ) ) .
	manualset3
85590	1	398352	5	NULL	NULL	0	NULL	elevated mutation levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show elevated mutation levels in single cells from Drosophila melanogaster S2 and mouse embryonic fibroblast populations after treatment with the powerful mutagen N-ethyl-N-nitrosourea .
	manualset3
85591	2	398352	5	NULL	NULL	NULL	NULL	single cells from Drosophila melanogaster S2	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we show elevated mutation levels in single cells from Drosophila melanogaster S2 and mouse embryonic fibroblast populations after treatment with the powerful mutagen N-ethyl-N-nitrosourea .
	manualset3
85592	3	398352	5	NULL	NULL	NULL	NULL	mouse embryonic fibroblast populations	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we show elevated mutation levels in single cells from Drosophila melanogaster S2 and mouse embryonic fibroblast populations after treatment with the powerful mutagen N-ethyl-N-nitrosourea .
	manualset3
85593	4	398352	5	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show elevated mutation levels in single cells from Drosophila melanogaster S2 and mouse embryonic fibroblast populations after treatment with the powerful mutagen N-ethyl-N-nitrosourea .
	manualset3
85594	5	398352	5	NULL	NULL	0	NULL	powerful mutagen N-ethyl-N-nitrosourea	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show elevated mutation levels in single cells from Drosophila melanogaster S2 and mouse embryonic fibroblast populations after treatment with the powerful mutagen N-ethyl-N-nitrosourea .
	manualset3
85595	1	398353	5	NULL	NULL	0	NULL	possession	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that , paradoxically , possession of the varepsilon4 allele confers a cognitive advantage on tasks mediated by the frontal lobe , and that young carriers of the varepsilon4 allele show larger cognitive benefit from procholinergic nicotinic stimulation .
	manualset3
85596	2	398353	5	NULL	NULL	0	NULL	varepsilon4 allele	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that , paradoxically , possession of the varepsilon4 allele confers a cognitive advantage on tasks mediated by the frontal lobe , and that young carriers of the varepsilon4 allele show larger cognitive benefit from procholinergic nicotinic stimulation .
	manualset3
85597	3	398353	5	NULL	NULL	0	NULL	cognitive advantage	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that , paradoxically , possession of the varepsilon4 allele confers a cognitive advantage on tasks mediated by the frontal lobe , and that young carriers of the varepsilon4 allele show larger cognitive benefit from procholinergic nicotinic stimulation .
	manualset3
85598	4	398353	5	NULL	NULL	0	NULL	frontal lobe	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that , paradoxically , possession of the varepsilon4 allele confers a cognitive advantage on tasks mediated by the frontal lobe , and that young carriers of the varepsilon4 allele show larger cognitive benefit from procholinergic nicotinic stimulation .
	manualset3
85599	5	398353	5	NULL	NULL	0	NULL	young carriers of the varepsilon4 allele	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that , paradoxically , possession of the varepsilon4 allele confers a cognitive advantage on tasks mediated by the frontal lobe , and that young carriers of the varepsilon4 allele show larger cognitive benefit from procholinergic nicotinic stimulation .
	manualset3
85600	6	398353	5	NULL	NULL	0	NULL	cognitive benefit	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that , paradoxically , possession of the varepsilon4 allele confers a cognitive advantage on tasks mediated by the frontal lobe , and that young carriers of the varepsilon4 allele show larger cognitive benefit from procholinergic nicotinic stimulation .
	manualset3
85601	7	398353	5	NULL	NULL	0	NULL	 procholinergic nicotinic stimulation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that , paradoxically , possession of the varepsilon4 allele confers a cognitive advantage on tasks mediated by the frontal lobe , and that young carriers of the varepsilon4 allele show larger cognitive benefit from procholinergic nicotinic stimulation .
	manualset3
86484	8	398353	5	NULL	NULL	0	NULL	tasks	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that , paradoxically , possession of the varepsilon4 allele confers a cognitive advantage on tasks mediated by the frontal lobe , and that young carriers of the varepsilon4 allele show larger cognitive benefit from procholinergic nicotinic stimulation .
	manualset3
85602	1	398354	5	NULL	NULL	0	NULL	viewing of natural scenes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that during viewing of natural scenes , microscopic eye movements carry out a crucial information-processing step : they remove predictable correlations in natural scenes by equalizing the spatial power of the retinal image within the frequency range of ganglion cells ' peak sensitivity .
	manualset3
85603	2	398354	5	NULL	NULL	0	NULL	microscopic eye movements	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that during viewing of natural scenes , microscopic eye movements carry out a crucial information-processing step : they remove predictable correlations in natural scenes by equalizing the spatial power of the retinal image within the frequency range of ganglion cells ' peak sensitivity .
	manualset3
85604	3	398354	5	NULL	NULL	NULL	NULL	information-processing step	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we show that during viewing of natural scenes , microscopic eye movements carry out a crucial information-processing step : they remove predictable correlations in natural scenes by equalizing the spatial power of the retinal image within the frequency range of ganglion cells ' peak sensitivity .
	manualset3
85605	4	398354	5	NULL	NULL	NULL	NULL	predictable correlations	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we show that during viewing of natural scenes , microscopic eye movements carry out a crucial information-processing step : they remove predictable correlations in natural scenes by equalizing the spatial power of the retinal image within the frequency range of ganglion cells ' peak sensitivity .
	manualset3
86398	5	398354	5	NULL	NULL	0	NULL	spatial power of the retinal image	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that during viewing of natural scenes , microscopic eye movements carry out a crucial information-processing step : they remove predictable correlations in natural scenes by equalizing the spatial power of the retinal image within the frequency range of ganglion cells ' peak sensitivity .
	manualset3
86399	6	398354	5	NULL	NULL	0	NULL	frequency range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that during viewing of natural scenes , microscopic eye movements carry out a crucial information-processing step : they remove predictable correlations in natural scenes by equalizing the spatial power of the retinal image within the frequency range of ganglion cells ' peak sensitivity .
	manualset3
86400	7	398354	5	NULL	NULL	0	NULL	ganglion cells ' peak sensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that during viewing of natural scenes , microscopic eye movements carry out a crucial information-processing step : they remove predictable correlations in natural scenes by equalizing the spatial power of the retinal image within the frequency range of ganglion cells ' peak sensitivity .
	manualset3
85626	1	398355	5	NULL	NULL	NULL	NULL	endogenous mp53 knockdown	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we show that endogenous mp53 knockdown enhanced cell migration and phosphorylation of ERK in DU145 prostate cancer cells .
	manualset3
85627	3	398355	5	NULL	NULL	NULL	NULL	phosphorylation of ERK	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we show that endogenous mp53 knockdown enhanced cell migration and phosphorylation of ERK in DU145 prostate cancer cells .
	manualset3
85628	4	398355	5	NULL	NULL	NULL	NULL	DU145 prostate cancer cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we show that endogenous mp53 knockdown enhanced cell migration and phosphorylation of ERK in DU145 prostate cancer cells .
	manualset3
85629	2	398355	5	NULL	NULL	0	NULL	cell migration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that endogenous mp53 knockdown enhanced cell migration and phosphorylation of ERK in DU145 prostate cancer cells .
	manualset3
85607	1	398356	5	NULL	NULL	NULL	NULL	mPTP opening	AnatomicalPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we show that mPTP opening acts as an initiating event to stimulate Bax translocation to mitochondria .
	manualset3
85608	2	398356	5	NULL	NULL	0	NULL	initiating event	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that mPTP opening acts as an initiating event to stimulate Bax translocation to mitochondria .
	manualset3
85609	3	398356	5	NULL	NULL	0	NULL	Bax translocation to mitochondria	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that mPTP opening acts as an initiating event to stimulate Bax translocation to mitochondria .
	manualset3
85610	1	398357	5	NULL	NULL	0	NULL	mda-7	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that mda-7 and IL-19 bind to the previously described IL-20R complex , composed by cytokine receptor family 2-8 / IL-20Ralpha and DIRS1/IL -20 Rbeta ( type I IL-20R ) .
	manualset3
85611	2	398357	5	NULL	NULL	0	NULL	IL-19	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that mda-7 and IL-19 bind to the previously described IL-20R complex , composed by cytokine receptor family 2-8 / IL-20Ralpha and DIRS1/IL -20 Rbeta ( type I IL-20R ) .
	manualset3
85612	3	398357	5	NULL	NULL	0	NULL	IL-20R complex	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that mda-7 and IL-19 bind to the previously described IL-20R complex , composed by cytokine receptor family 2-8 / IL-20Ralpha and DIRS1/IL -20 Rbeta ( type I IL-20R ) .
	manualset3
85613	4	398357	5	NULL	NULL	0	NULL	cytokine receptor family 2-8 / IL-20Ralpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that mda-7 and IL-19 bind to the previously described IL-20R complex , composed by cytokine receptor family 2-8 / IL-20Ralpha and DIRS1/IL -20 Rbeta ( type I IL-20R ) .
	manualset3
85614	5	398357	5	NULL	NULL	0	NULL	DIRS1/IL -20 Rbeta ( type I IL-20R )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that mda-7 and IL-19 bind to the previously described IL-20R complex , composed by cytokine receptor family 2-8 / IL-20Ralpha and DIRS1/IL -20 Rbeta ( type I IL-20R ) .
	manualset3
85615	1	398358	5	NULL	NULL	0	NULL	semaphorin 3A ( Sema3A ) expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that semaphorin 3A ( Sema3A ) expression overcomes the proinvasive and prometastatic resistance observed upon angiogenesis reduction by the small-molecule tyrosine inhibitor sunitinib in both pancreatic neuroendocrine tumors ( PNETs ) in RIP-Tag2 mice and cervical carcinomas in HPV16/E2 mice .
	manualset3
85616	2	398358	5	NULL	NULL	NULL	NULL	proinvasive and prometastatic resistance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we show that semaphorin 3A ( Sema3A ) expression overcomes the proinvasive and prometastatic resistance observed upon angiogenesis reduction by the small-molecule tyrosine inhibitor sunitinib in both pancreatic neuroendocrine tumors ( PNETs ) in RIP-Tag2 mice and cervical carcinomas in HPV16/E2 mice .
	manualset3
85617	3	398358	5	NULL	NULL	NULL	NULL	angiogenesis reduction	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we show that semaphorin 3A ( Sema3A ) expression overcomes the proinvasive and prometastatic resistance observed upon angiogenesis reduction by the small-molecule tyrosine inhibitor sunitinib in both pancreatic neuroendocrine tumors ( PNETs ) in RIP-Tag2 mice and cervical carcinomas in HPV16/E2 mice .
	manualset3
85618	4	398358	5	NULL	NULL	0	NULL	 small-molecule tyrosine inhibitor sunitinib	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that semaphorin 3A ( Sema3A ) expression overcomes the proinvasive and prometastatic resistance observed upon angiogenesis reduction by the small-molecule tyrosine inhibitor sunitinib in both pancreatic neuroendocrine tumors ( PNETs ) in RIP-Tag2 mice and cervical carcinomas in HPV16/E2 mice .
	manualset3
85619	5	398358	5	NULL	NULL	0	NULL	pancreatic neuroendocrine tumors ( PNETs )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that semaphorin 3A ( Sema3A ) expression overcomes the proinvasive and prometastatic resistance observed upon angiogenesis reduction by the small-molecule tyrosine inhibitor sunitinib in both pancreatic neuroendocrine tumors ( PNETs ) in RIP-Tag2 mice and cervical carcinomas in HPV16/E2 mice .
	manualset3
85620	6	398358	5	NULL	NULL	0	NULL	RIP-Tag2 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that semaphorin 3A ( Sema3A ) expression overcomes the proinvasive and prometastatic resistance observed upon angiogenesis reduction by the small-molecule tyrosine inhibitor sunitinib in both pancreatic neuroendocrine tumors ( PNETs ) in RIP-Tag2 mice and cervical carcinomas in HPV16/E2 mice .
	manualset3
85621	7	398358	5	NULL	NULL	0	NULL	cervical carcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that semaphorin 3A ( Sema3A ) expression overcomes the proinvasive and prometastatic resistance observed upon angiogenesis reduction by the small-molecule tyrosine inhibitor sunitinib in both pancreatic neuroendocrine tumors ( PNETs ) in RIP-Tag2 mice and cervical carcinomas in HPV16/E2 mice .
	manualset3
85622	8	398358	5	NULL	NULL	0	NULL	HPV16/E2 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that semaphorin 3A ( Sema3A ) expression overcomes the proinvasive and prometastatic resistance observed upon angiogenesis reduction by the small-molecule tyrosine inhibitor sunitinib in both pancreatic neuroendocrine tumors ( PNETs ) in RIP-Tag2 mice and cervical carcinomas in HPV16/E2 mice .
	manualset3
85623	1	398359	5	NULL	NULL	0	NULL	catenin pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that the - catenin pathway is active in the limb-forming area in mouse embryos .
	manualset3
85624	2	398359	5	NULL	NULL	0	NULL	limb-forming area	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that the - catenin pathway is active in the limb-forming area in mouse embryos .
	manualset3
85625	3	398359	5	NULL	NULL	0	NULL	mouse embryos	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that the - catenin pathway is active in the limb-forming area in mouse embryos .
	manualset3
85660	1	398360	5	NULL	NULL	0	NULL	HSCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that the HSCs from the embryonic aorta are the most potently supported HSCs in UG stromal clone co-cultures and that contact is required for the maintenance and expansion of embryo-derived HSCs .
	manualset3
85661	2	398360	5	NULL	NULL	0	NULL	embryonic aorta	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that the HSCs from the embryonic aorta are the most potently supported HSCs in UG stromal clone co-cultures and that contact is required for the maintenance and expansion of embryo-derived HSCs .
	manualset3
85662	3	398360	5	NULL	NULL	0	NULL	HSCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that the HSCs from the embryonic aorta are the most potently supported HSCs in UG stromal clone co-cultures and that contact is required for the maintenance and expansion of embryo-derived HSCs .
	manualset3
85664	4	398360	5	NULL	NULL	0	NULL	UG stromal clone co-cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that the HSCs from the embryonic aorta are the most potently supported HSCs in UG stromal clone co-cultures and that contact is required for the maintenance and expansion of embryo-derived HSCs .
	manualset3
85666	5	398360	5	NULL	NULL	0	NULL	maintenance and expansion of embryo-derived HSCs	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that the HSCs from the embryonic aorta are the most potently supported HSCs in UG stromal clone co-cultures and that contact is required for the maintenance and expansion of embryo-derived HSCs .
	manualset3
85670	1	398361	5	NULL	NULL	0	NULL	allogeneic stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that the allogeneic stimulation also induces the appearance in the low molecular weight fraction of the serum ( 1000-110 , 000 MW ) of an inhibitor which blocks the PBA activity of the complex without affecting the PBA activity of LPS or dextran sulphate .
	manualset3
85674	2	398361	5	NULL	NULL	0	NULL	appearance	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that the allogeneic stimulation also induces the appearance in the low molecular weight fraction of the serum ( 1000-110 , 000 MW ) of an inhibitor which blocks the PBA activity of the complex without affecting the PBA activity of LPS or dextran sulphate .
	manualset3
85675	3	398361	5	NULL	NULL	0	NULL	low molecular weight fraction of the serum ( 1000-110 , 000 MW )	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that the allogeneic stimulation also induces the appearance in the low molecular weight fraction of the serum ( 1000-110 , 000 MW ) of an inhibitor which blocks the PBA activity of the complex without affecting the PBA activity of LPS or dextran sulphate .
	manualset3
85677	4	398361	5	NULL	NULL	0	NULL	inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that the allogeneic stimulation also induces the appearance in the low molecular weight fraction of the serum ( 1000-110 , 000 MW ) of an inhibitor which blocks the PBA activity of the complex without affecting the PBA activity of LPS or dextran sulphate .
	manualset3
85679	5	398361	5	NULL	NULL	0	NULL	PBA activity of the complex	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that the allogeneic stimulation also induces the appearance in the low molecular weight fraction of the serum ( 1000-110 , 000 MW ) of an inhibitor which blocks the PBA activity of the complex without affecting the PBA activity of LPS or dextran sulphate .
	manualset3
85697	6	398361	5	NULL	NULL	0	NULL	PBA activity of LPS or dextran sulphate	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that the allogeneic stimulation also induces the appearance in the low molecular weight fraction of the serum ( 1000-110 , 000 MW ) of an inhibitor which blocks the PBA activity of the complex without affecting the PBA activity of LPS or dextran sulphate .
	manualset3
85698	1	398362	5	NULL	NULL	0	NULL	Surgical indications	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Surgical indications in ileus ) .
	manualset3
85699	2	398362	5	NULL	NULL	0	NULL	ileus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Surgical indications in ileus ) .
	manualset3
85939	1	398363	5	NULL	NULL	0	NULL	coexpression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that the coexpression of another HCMV glycoprotein , gO , with gH/gL in human fibroblasts interferes with HCMV entry into fibroblasts but not epithelial cells .
	manualset3
85940	2	398363	5	NULL	NULL	0	NULL	HCMV glycoprotein , gO	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that the coexpression of another HCMV glycoprotein , gO , with gH/gL in human fibroblasts interferes with HCMV entry into fibroblasts but not epithelial cells .
	manualset3
85941	3	398363	5	NULL	NULL	0	NULL	gH/gL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that the coexpression of another HCMV glycoprotein , gO , with gH/gL in human fibroblasts interferes with HCMV entry into fibroblasts but not epithelial cells .
	manualset3
85942	4	398363	5	NULL	NULL	0	NULL	human fibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that the coexpression of another HCMV glycoprotein , gO , with gH/gL in human fibroblasts interferes with HCMV entry into fibroblasts but not epithelial cells .
	manualset3
85943	5	398363	5	NULL	NULL	0	NULL	HCMV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that the coexpression of another HCMV glycoprotein , gO , with gH/gL in human fibroblasts interferes with HCMV entry into fibroblasts but not epithelial cells .
	manualset3
85944	6	398363	5	NULL	NULL	0	NULL	fibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that the coexpression of another HCMV glycoprotein , gO , with gH/gL in human fibroblasts interferes with HCMV entry into fibroblasts but not epithelial cells .
	manualset3
85945	7	398363	5	NULL	NULL	0	NULL	epithelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that the coexpression of another HCMV glycoprotein , gO , with gH/gL in human fibroblasts interferes with HCMV entry into fibroblasts but not epithelial cells .
	manualset3
85946	1	398364	5	NULL	NULL	0	NULL	decreased FA synthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that the decreased FA synthesis in liver is balanced by an equal increase in nonhepatic tissues , primarily adipose tissue .
	manualset3
85947	2	398364	5	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that the decreased FA synthesis in liver is balanced by an equal increase in nonhepatic tissues , primarily adipose tissue .
	manualset3
85948	3	398364	5	NULL	NULL	0	NULL	nonhepatic tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that the decreased FA synthesis in liver is balanced by an equal increase in nonhepatic tissues , primarily adipose tissue .
	manualset3
85949	4	398364	5	NULL	NULL	0	NULL	adipose tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that the decreased FA synthesis in liver is balanced by an equal increase in nonhepatic tissues , primarily adipose tissue .
	manualset3
85950	1	398365	5	NULL	NULL	0	NULL	interleukin-1 receptor-associated kinase ( IRAK ) / Pelle-like kinase gene SHORT SUSPENSOR ( SSP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that the interleukin-1 receptor-associated kinase ( IRAK ) / Pelle-like kinase gene SHORT SUSPENSOR ( SSP ) regulates this pathway through a previously unknown parent-of-origin effect .
	manualset3
85951	2	398365	5	NULL	NULL	0	NULL	pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that the interleukin-1 receptor-associated kinase ( IRAK ) / Pelle-like kinase gene SHORT SUSPENSOR ( SSP ) regulates this pathway through a previously unknown parent-of-origin effect .
	manualset3
85952	3	398365	5	NULL	NULL	0	NULL	parent-of-origin effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we show that the interleukin-1 receptor-associated kinase ( IRAK ) / Pelle-like kinase gene SHORT SUSPENSOR ( SSP ) regulates this pathway through a previously unknown parent-of-origin effect .
	manualset3
85953	1	398366	5	NULL	NULL	0	NULL	gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we sought to identify gene expression in the medial prefrontal cortex ( mPFC ) of mice associated with PPI using a laser microdissection and microarray analysis-based approach .
	manualset3
85954	2	398366	5	NULL	NULL	0	NULL	medial prefrontal cortex ( mPFC )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we sought to identify gene expression in the medial prefrontal cortex ( mPFC ) of mice associated with PPI using a laser microdissection and microarray analysis-based approach .
	manualset3
85955	3	398366	5	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we sought to identify gene expression in the medial prefrontal cortex ( mPFC ) of mice associated with PPI using a laser microdissection and microarray analysis-based approach .
	manualset3
85956	4	398366	5	NULL	NULL	0	NULL	PPI	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we sought to identify gene expression in the medial prefrontal cortex ( mPFC ) of mice associated with PPI using a laser microdissection and microarray analysis-based approach .
	manualset3
85957	5	398366	5	NULL	NULL	0	NULL	laser microdissection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we sought to identify gene expression in the medial prefrontal cortex ( mPFC ) of mice associated with PPI using a laser microdissection and microarray analysis-based approach .
	manualset3
85958	6	398366	5	NULL	NULL	0	NULL	microarray analysis-based approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we sought to identify gene expression in the medial prefrontal cortex ( mPFC ) of mice associated with PPI using a laser microdissection and microarray analysis-based approach .
	manualset3
85959	1	398367	5	NULL	NULL	0	NULL	intracellular localisation of siRNA and Argonaute 2 ( Ago2 )	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we studied the intracellular localisation of siRNA and Argonaute 2 ( Ago2 ) , the major component of the RNA interference ( RNAi ) machinery , by density gradient centrifugation and fluorescence microscopy after PS-stimulated delivery or transfection with Lipofectamine 2000 .
	manualset3
85960	2	398367	5	NULL	NULL	0	NULL	RNA interference ( RNAi ) machinery	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we studied the intracellular localisation of siRNA and Argonaute 2 ( Ago2 ) , the major component of the RNA interference ( RNAi ) machinery , by density gradient centrifugation and fluorescence microscopy after PS-stimulated delivery or transfection with Lipofectamine 2000 .
	manualset3
85961	3	398367	5	NULL	NULL	0	NULL	density gradient centrifugation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we studied the intracellular localisation of siRNA and Argonaute 2 ( Ago2 ) , the major component of the RNA interference ( RNAi ) machinery , by density gradient centrifugation and fluorescence microscopy after PS-stimulated delivery or transfection with Lipofectamine 2000 .
	manualset3
85962	4	398367	5	NULL	NULL	0	NULL	fluorescence microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we studied the intracellular localisation of siRNA and Argonaute 2 ( Ago2 ) , the major component of the RNA interference ( RNAi ) machinery , by density gradient centrifugation and fluorescence microscopy after PS-stimulated delivery or transfection with Lipofectamine 2000 .
	manualset3
85963	5	398367	5	NULL	NULL	0	NULL	PS-stimulated delivery	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we studied the intracellular localisation of siRNA and Argonaute 2 ( Ago2 ) , the major component of the RNA interference ( RNAi ) machinery , by density gradient centrifugation and fluorescence microscopy after PS-stimulated delivery or transfection with Lipofectamine 2000 .
	manualset3
85964	6	398367	5	NULL	NULL	0	NULL	transfection with Lipofectamine 2000	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we studied the intracellular localisation of siRNA and Argonaute 2 ( Ago2 ) , the major component of the RNA interference ( RNAi ) machinery , by density gradient centrifugation and fluorescence microscopy after PS-stimulated delivery or transfection with Lipofectamine 2000 .
	manualset3
85965	1	398368	5	NULL	NULL	0	NULL	 hypothesis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we test the hypothesis that BMSCs suppress immune responses by Fas-mediated apoptosis of activated lymphocytes and find both Fas and FasL expression by primary BMSCs .
	manualset3
85966	2	398368	5	NULL	NULL	0	NULL	BMSCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we test the hypothesis that BMSCs suppress immune responses by Fas-mediated apoptosis of activated lymphocytes and find both Fas and FasL expression by primary BMSCs .
	manualset3
85967	3	398368	5	NULL	NULL	0	NULL	immune responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we test the hypothesis that BMSCs suppress immune responses by Fas-mediated apoptosis of activated lymphocytes and find both Fas and FasL expression by primary BMSCs .
	manualset3
85968	4	398368	5	NULL	NULL	0	NULL	Fas-mediated apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we test the hypothesis that BMSCs suppress immune responses by Fas-mediated apoptosis of activated lymphocytes and find both Fas and FasL expression by primary BMSCs .
	manualset3
85969	5	398368	5	NULL	NULL	0	NULL	activated lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we test the hypothesis that BMSCs suppress immune responses by Fas-mediated apoptosis of activated lymphocytes and find both Fas and FasL expression by primary BMSCs .
	manualset3
85970	6	398368	5	NULL	NULL	0	NULL	Fas and FasL expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we test the hypothesis that BMSCs suppress immune responses by Fas-mediated apoptosis of activated lymphocytes and find both Fas and FasL expression by primary BMSCs .
	manualset3
85971	7	398368	5	NULL	NULL	0	NULL	primary BMSCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we test the hypothesis that BMSCs suppress immune responses by Fas-mediated apoptosis of activated lymphocytes and find both Fas and FasL expression by primary BMSCs .
	manualset3
85972	1	398369	5	NULL	NULL	0	NULL	NIRS	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we tested the applicability of imaging NIRS to the discrimination of cryptic species by using the ants Tetramorium caespitum and T. impurum .
	manualset3
85973	2	398369	5	NULL	NULL	0	NULL	discrimination of cryptic species	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we tested the applicability of imaging NIRS to the discrimination of cryptic species by using the ants Tetramorium caespitum and T. impurum .
	manualset3
85974	3	398369	5	NULL	NULL	0	NULL	ants Tetramorium caespitum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we tested the applicability of imaging NIRS to the discrimination of cryptic species by using the ants Tetramorium caespitum and T. impurum .
	manualset3
85975	4	398369	5	NULL	NULL	0	NULL	T. impurum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we tested the applicability of imaging NIRS to the discrimination of cryptic species by using the ants Tetramorium caespitum and T. impurum .
	manualset3
85976	1	398370	5	NULL	NULL	0	NULL	 rodent model	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we use a rodent model of an aversive cue-induced cessation of feeding .
	manualset3
85977	2	398370	5	NULL	NULL	0	NULL	aversive cue-induced cessation of feeding	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we use a rodent model of an aversive cue-induced cessation of feeding .
	manualset3
85978	1	398371	5	NULL	NULL	NULL	NULL	acute in vivo genetic manipulation of synaptic proteins	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we use acute in vivo genetic manipulation of synaptic proteins to investigate the molecular basis for presynaptic long-term potentiation ( LTP ) at hippocampal mossy fiber synapses .
	manualset3
85979	2	398371	5	NULL	NULL	0	NULL	presynaptic long-term potentiation ( LTP )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we use acute in vivo genetic manipulation of synaptic proteins to investigate the molecular basis for presynaptic long-term potentiation ( LTP ) at hippocampal mossy fiber synapses .
	manualset3
85980	3	398371	5	NULL	NULL	0	NULL	hippocampal mossy fiber synapses	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we use acute in vivo genetic manipulation of synaptic proteins to investigate the molecular basis for presynaptic long-term potentiation ( LTP ) at hippocampal mossy fiber synapses .
	manualset3
85981	1	398372	5	NULL	NULL	0	NULL	chemical probing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we use chemical probing to show that interaction sites with the 40S subunit and eIF3 are conserved between HCV and HCV-like IRESs .
	manualset3
85982	2	398372	5	NULL	NULL	NULL	NULL	interaction sites with the 40S subunit and eIF3	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we use chemical probing to show that interaction sites with the 40S subunit and eIF3 are conserved between HCV and HCV-like IRESs .
	manualset3
85983	3	398372	5	NULL	NULL	NULL	NULL	HCV	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we use chemical probing to show that interaction sites with the 40S subunit and eIF3 are conserved between HCV and HCV-like IRESs .
	manualset3
87582	4	398372	5	NULL	NULL	0	NULL	HCV-like IRESs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we use chemical probing to show that interaction sites with the 40S subunit and eIF3 are conserved between HCV and HCV-like IRESs .
	manualset3
85984	1	398373	5	NULL	NULL	NULL	NULL	Surgical protocol	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Surgical protocol and intraoperative considerations in interventions on the testis ) .
	manualset3
85985	3	398373	5	NULL	NULL	NULL	NULL	interventions on the testis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Surgical protocol and intraoperative considerations in interventions on the testis ) .
	manualset3
86485	2	398373	5	NULL	NULL	NULL	NULL	intraoperative considerations	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Surgical protocol and intraoperative considerations in interventions on the testis ) .
	manualset3
85986	1	398374	5	NULL	NULL	0	NULL	precursor ion scanning MS	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we use precursor ion scanning MS to identify five previously unknown sites in MSK1 : Thr630 , Ser647 , Ser657 , Ser695 and Thr700 .
	manualset3
85987	2	398374	5	NULL	NULL	0	NULL	MSK1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we use precursor ion scanning MS to identify five previously unknown sites in MSK1 : Thr630 , Ser647 , Ser657 , Ser695 and Thr700 .
	manualset3
85988	3	398374	5	NULL	NULL	0	NULL	Thr630	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we use precursor ion scanning MS to identify five previously unknown sites in MSK1 : Thr630 , Ser647 , Ser657 , Ser695 and Thr700 .
	manualset3
85989	4	398374	5	NULL	NULL	0	NULL	Ser647	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we use precursor ion scanning MS to identify five previously unknown sites in MSK1 : Thr630 , Ser647 , Ser657 , Ser695 and Thr700 .
	manualset3
85990	5	398374	5	NULL	NULL	0	NULL	Ser657	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we use precursor ion scanning MS to identify five previously unknown sites in MSK1 : Thr630 , Ser647 , Ser657 , Ser695 and Thr700 .
	manualset3
85991	6	398374	5	NULL	NULL	0	NULL	Ser695	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we use precursor ion scanning MS to identify five previously unknown sites in MSK1 : Thr630 , Ser647 , Ser657 , Ser695 and Thr700 .
	manualset3
85992	7	398374	5	NULL	NULL	0	NULL	Thr700	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we use precursor ion scanning MS to identify five previously unknown sites in MSK1 : Thr630 , Ser647 , Ser657 , Ser695 and Thr700 .
	manualset3
85993	2	398375	5	NULL	NULL	NULL	NULL	non-cellular solid-state compartment	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we will focus on studies concerning a common theme , which is the central importance of the non-cellular solid-state compartment as a master regulator of the malignant phenotype .
	manualset3
85994	3	398375	5	NULL	NULL	NULL	NULL	master regulator	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we will focus on studies concerning a common theme , which is the central importance of the non-cellular solid-state compartment as a master regulator of the malignant phenotype .
	manualset3
85995	4	398375	5	NULL	NULL	NULL	NULL	malignant phenotype	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here , we will focus on studies concerning a common theme , which is the central importance of the non-cellular solid-state compartment as a master regulator of the malignant phenotype .
	manualset3
86401	1	398375	5	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we will focus on studies concerning a common theme , which is the central importance of the non-cellular solid-state compartment as a master regulator of the malignant phenotype .
	manualset3
85996	1	398376	5	NULL	NULL	NULL	NULL	physiological field , immunology	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here I show that one physiological field , immunology , offers a theory that makes possible a biological individuation based on physiological grounds .
	manualset3
85997	2	398376	5	NULL	NULL	0	NULL	theory	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Here I show that one physiological field , immunology , offers a theory that makes possible a biological individuation based on physiological grounds .
	manualset3
86340	3	398376	5	NULL	NULL	0	NULL	biological individuation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here I show that one physiological field , immunology , offers a theory that makes possible a biological individuation based on physiological grounds .
	manualset3
86402	4	398376	5	NULL	NULL	0	NULL	physiological grounds	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here I show that one physiological field , immunology , offers a theory that makes possible a biological individuation based on physiological grounds .
	manualset3
85998	1	398377	5	NULL	NULL	0	NULL	chimeric model system	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here a chimeric model system consisting of human cytochrome P450 3A4 and the soluble reductase domain of CYP102A1 from Bacillus megaterium ( BMR ) is used to study the relationship between electron transfer and the coupling efficiency in substrate monoxygenation .
	manualset3
85999	2	398377	5	NULL	NULL	0	NULL	human cytochrome P450 3A4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here a chimeric model system consisting of human cytochrome P450 3A4 and the soluble reductase domain of CYP102A1 from Bacillus megaterium ( BMR ) is used to study the relationship between electron transfer and the coupling efficiency in substrate monoxygenation .
	manualset3
86000	3	398377	5	NULL	NULL	0	NULL	soluble reductase domain of CYP102A1	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here a chimeric model system consisting of human cytochrome P450 3A4 and the soluble reductase domain of CYP102A1 from Bacillus megaterium ( BMR ) is used to study the relationship between electron transfer and the coupling efficiency in substrate monoxygenation .
	manualset3
86001	4	398377	5	NULL	NULL	0	NULL	Bacillus megaterium ( BMR )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here a chimeric model system consisting of human cytochrome P450 3A4 and the soluble reductase domain of CYP102A1 from Bacillus megaterium ( BMR ) is used to study the relationship between electron transfer and the coupling efficiency in substrate monoxygenation .
	manualset3
86002	5	398377	5	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Here a chimeric model system consisting of human cytochrome P450 3A4 and the soluble reductase domain of CYP102A1 from Bacillus megaterium ( BMR ) is used to study the relationship between electron transfer and the coupling efficiency in substrate monoxygenation .
	manualset3
86003	6	398377	5	NULL	NULL	NULL	NULL	electron transfer	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here a chimeric model system consisting of human cytochrome P450 3A4 and the soluble reductase domain of CYP102A1 from Bacillus megaterium ( BMR ) is used to study the relationship between electron transfer and the coupling efficiency in substrate monoxygenation .
	manualset3
86486	7	398377	5	NULL	NULL	0	NULL	coupling efficiency	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here a chimeric model system consisting of human cytochrome P450 3A4 and the soluble reductase domain of CYP102A1 from Bacillus megaterium ( BMR ) is used to study the relationship between electron transfer and the coupling efficiency in substrate monoxygenation .
	manualset3
86487	8	398377	5	NULL	NULL	0	NULL	 substrate monoxygenation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here a chimeric model system consisting of human cytochrome P450 3A4 and the soluble reductase domain of CYP102A1 from Bacillus megaterium ( BMR ) is used to study the relationship between electron transfer and the coupling efficiency in substrate monoxygenation .
	manualset3
86004	1	398378	5	NULL	NULL	0	NULL	transparietojejunal endoscopic investigation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here a transparietojejunal endoscopic investigation is proposed that permits direct sight of the anastomosis , biliary sampling for cultural examination and dilatative type therapeutic maneuvers , biopsies or extractions of residual stones from the bile ways that would not otherwise be possible without further surgery .
	manualset3
86005	2	398378	5	NULL	NULL	NULL	NULL	direct sight of the anastomosis	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here a transparietojejunal endoscopic investigation is proposed that permits direct sight of the anastomosis , biliary sampling for cultural examination and dilatative type therapeutic maneuvers , biopsies or extractions of residual stones from the bile ways that would not otherwise be possible without further surgery .
	manualset3
86006	3	398378	5	NULL	NULL	0	NULL	biliary sampling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here a transparietojejunal endoscopic investigation is proposed that permits direct sight of the anastomosis , biliary sampling for cultural examination and dilatative type therapeutic maneuvers , biopsies or extractions of residual stones from the bile ways that would not otherwise be possible without further surgery .
	manualset3
86007	4	398378	5	NULL	NULL	0	NULL	cultural examination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here a transparietojejunal endoscopic investigation is proposed that permits direct sight of the anastomosis , biliary sampling for cultural examination and dilatative type therapeutic maneuvers , biopsies or extractions of residual stones from the bile ways that would not otherwise be possible without further surgery .
	manualset3
86008	5	398378	5	NULL	NULL	0	NULL	dilatative type therapeutic maneuvers	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Here a transparietojejunal endoscopic investigation is proposed that permits direct sight of the anastomosis , biliary sampling for cultural examination and dilatative type therapeutic maneuvers , biopsies or extractions of residual stones from the bile ways that would not otherwise be possible without further surgery .
	manualset3
86009	6	398378	5	NULL	NULL	0	NULL	biopsies or extractions of residual stones from the bile	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Here a transparietojejunal endoscopic investigation is proposed that permits direct sight of the anastomosis , biliary sampling for cultural examination and dilatative type therapeutic maneuvers , biopsies or extractions of residual stones from the bile ways that would not otherwise be possible without further surgery .
	manualset3
86010	7	398378	5	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Here a transparietojejunal endoscopic investigation is proposed that permits direct sight of the anastomosis , biliary sampling for cultural examination and dilatative type therapeutic maneuvers , biopsies or extractions of residual stones from the bile ways that would not otherwise be possible without further surgery .
	manualset3
86011	1	398379	5	NULL	NULL	0	NULL	unusual complication of the treatment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here an unusual complication of the treatment is reported : multiple tender subcutaneous nodules developed where the catgut was embedded over the lower abdomen and both medial thighs 1 month after treatment .
	manualset3
86020	2	398379	5	NULL	NULL	NULL	NULL	multiple tender subcutaneous nodules	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here an unusual complication of the treatment is reported : multiple tender subcutaneous nodules developed where the catgut was embedded over the lower abdomen and both medial thighs 1 month after treatment .
	manualset3
86021	3	398379	5	NULL	NULL	NULL	NULL	catgut	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here an unusual complication of the treatment is reported : multiple tender subcutaneous nodules developed where the catgut was embedded over the lower abdomen and both medial thighs 1 month after treatment .
	manualset3
86028	4	398379	5	NULL	NULL	0	NULL	lower abdomen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here an unusual complication of the treatment is reported : multiple tender subcutaneous nodules developed where the catgut was embedded over the lower abdomen and both medial thighs 1 month after treatment .
	manualset3
86032	5	398379	5	NULL	NULL	0	NULL	medial thighs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here an unusual complication of the treatment is reported : multiple tender subcutaneous nodules developed where the catgut was embedded over the lower abdomen and both medial thighs 1 month after treatment .
	manualset3
86033	6	398379	5	NULL	NULL	0	NULL	1 month after treatment	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Here an unusual complication of the treatment is reported : multiple tender subcutaneous nodules developed where the catgut was embedded over the lower abdomen and both medial thighs 1 month after treatment .
	manualset3
86036	1	398380	5	NULL	NULL	0	NULL	ARABIDOPSIS THALIANA HOMEOBOX GENE1 ( ATH1 ) gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Here it is reported that the ARABIDOPSIS THALIANA HOMEOBOX GENE1 ( ATH1 ) gene , which belongs to the BELL1-like homeodomain gene family , is a new member participating in regulating pedicel orientation in the class-I KNOX network .
	manualset3
86037	2	398380	5	NULL	NULL	0	NULL	BELL1-like homeodomain gene family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Here it is reported that the ARABIDOPSIS THALIANA HOMEOBOX GENE1 ( ATH1 ) gene , which belongs to the BELL1-like homeodomain gene family , is a new member participating in regulating pedicel orientation in the class-I KNOX network .
	manualset3
86038	3	398380	5	NULL	NULL	0	NULL	new member	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Here it is reported that the ARABIDOPSIS THALIANA HOMEOBOX GENE1 ( ATH1 ) gene , which belongs to the BELL1-like homeodomain gene family , is a new member participating in regulating pedicel orientation in the class-I KNOX network .
	manualset3
86039	4	398380	5	NULL	NULL	0	NULL	pedicel orientation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here it is reported that the ARABIDOPSIS THALIANA HOMEOBOX GENE1 ( ATH1 ) gene , which belongs to the BELL1-like homeodomain gene family , is a new member participating in regulating pedicel orientation in the class-I KNOX network .
	manualset3
86040	5	398380	5	NULL	NULL	0	NULL	class-I KNOX network	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here it is reported that the ARABIDOPSIS THALIANA HOMEOBOX GENE1 ( ATH1 ) gene , which belongs to the BELL1-like homeodomain gene family , is a new member participating in regulating pedicel orientation in the class-I KNOX network .
	manualset3
86041	1	398381	5	NULL	NULL	0	NULL	Xa21 homologs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we attempted to determine the existence of Xa21 homologs in other wild rice species and rice cultivars and the sequence differences between the homologs .
	manualset3
86042	2	398381	5	NULL	NULL	0	NULL	wild rice species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we attempted to determine the existence of Xa21 homologs in other wild rice species and rice cultivars and the sequence differences between the homologs .
	manualset3
86043	3	398381	5	NULL	NULL	0	NULL	rice cultivars	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we attempted to determine the existence of Xa21 homologs in other wild rice species and rice cultivars and the sequence differences between the homologs .
	manualset3
86044	4	398381	5	NULL	NULL	0	NULL	sequence differences between the homologs	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we attempted to determine the existence of Xa21 homologs in other wild rice species and rice cultivars and the sequence differences between the homologs .
	manualset3
86488	5	398381	5	NULL	NULL	0	NULL	existence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we attempted to determine the existence of Xa21 homologs in other wild rice species and rice cultivars and the sequence differences between the homologs .
	manualset3
86048	1	398382	5	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we collated data from 331 experiments in 255 healthy volunteers over a 23-year period , in which subcutaneous abdominal adipose tissue metabolism was studied by measurements of arterio-venous differences after an overnight fast .
	manualset3
86050	2	398382	5	NULL	NULL	0	NULL	331 experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we collated data from 331 experiments in 255 healthy volunteers over a 23-year period , in which subcutaneous abdominal adipose tissue metabolism was studied by measurements of arterio-venous differences after an overnight fast .
	manualset3
86051	3	398382	5	NULL	NULL	0	NULL	255 healthy volunteers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we collated data from 331 experiments in 255 healthy volunteers over a 23-year period , in which subcutaneous abdominal adipose tissue metabolism was studied by measurements of arterio-venous differences after an overnight fast .
	manualset3
86052	4	398382	5	NULL	NULL	0	NULL	23-year period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we collated data from 331 experiments in 255 healthy volunteers over a 23-year period , in which subcutaneous abdominal adipose tissue metabolism was studied by measurements of arterio-venous differences after an overnight fast .
	manualset3
86053	5	398382	5	NULL	NULL	0	NULL	subcutaneous abdominal adipose tissue metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we collated data from 331 experiments in 255 healthy volunteers over a 23-year period , in which subcutaneous abdominal adipose tissue metabolism was studied by measurements of arterio-venous differences after an overnight fast .
	manualset3
86054	6	398382	5	NULL	NULL	0	NULL	measurements of arterio-venous differences	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we collated data from 331 experiments in 255 healthy volunteers over a 23-year period , in which subcutaneous abdominal adipose tissue metabolism was studied by measurements of arterio-venous differences after an overnight fast .
	manualset3
86056	7	398382	5	NULL	NULL	0	NULL	overnight fast	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we collated data from 331 experiments in 255 healthy volunteers over a 23-year period , in which subcutaneous abdominal adipose tissue metabolism was studied by measurements of arterio-venous differences after an overnight fast .
	manualset3
86057	1	398383	5	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we deal with its role in the biosynthesis of the subclasses of ethanolamine - and choline-containing phosphoglycerides ( EPG , CPG , respectively ) .
	manualset3
86058	2	398383	5	NULL	NULL	0	NULL	 biosynthesis of the subclasses of ethanolamine	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we deal with its role in the biosynthesis of the subclasses of ethanolamine - and choline-containing phosphoglycerides ( EPG , CPG , respectively ) .
	manualset3
86059	3	398383	5	NULL	NULL	0	NULL	 biosynthesis of the subclasses of  choline-containing phosphoglycerides ( EPG , CPG , respectively )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we deal with its role in the biosynthesis of the subclasses of ethanolamine - and choline-containing phosphoglycerides ( EPG , CPG , respectively ) .
	manualset3
86098	1	398384	5	NULL	NULL	0	NULL	Surgical treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Surgical treatment of malignant neoplasms of the pancreatoduodenal zone ) .
	manualset3
86100	2	398384	5	NULL	NULL	0	NULL	malignant neoplasms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Surgical treatment of malignant neoplasms of the pancreatoduodenal zone ) .
	manualset3
86102	3	398384	5	NULL	NULL	0	NULL	pancreatoduodenal zone	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Surgical treatment of malignant neoplasms of the pancreatoduodenal zone ) .
	manualset3
86105	1	398385	5	NULL	NULL	0	NULL	input logic	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we define the input logic and transcriptional output of the stringent response in the oligotroph , Caulobacter crescentus .
	manualset3
86106	2	398385	5	NULL	NULL	0	NULL	transcriptional output	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we define the input logic and transcriptional output of the stringent response in the oligotroph , Caulobacter crescentus .
	manualset3
86107	3	398385	5	NULL	NULL	0	NULL	stringent response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we define the input logic and transcriptional output of the stringent response in the oligotroph , Caulobacter crescentus .
	manualset3
86108	4	398385	5	NULL	NULL	0	NULL	oligotroph	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we define the input logic and transcriptional output of the stringent response in the oligotroph , Caulobacter crescentus .
	manualset3
86109	5	398385	5	NULL	NULL	0	NULL	Caulobacter crescentus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we define the input logic and transcriptional output of the stringent response in the oligotroph , Caulobacter crescentus .
	manualset3
86147	1	398386	5	NULL	NULL	NULL	NULL	overexpression of NCAM ( CD56 )	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we demonstrate , that the overexpression of NCAM ( CD56 ) is specific for ischemic damage as compaired to other heart diseases including congestive cardiomyopathy , hypertrophic obstrutive cardiomyopathy , myocarditis and sarcoidosis .
	manualset3
86148	2	398386	5	NULL	NULL	0	NULL	ischemic damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we demonstrate , that the overexpression of NCAM ( CD56 ) is specific for ischemic damage as compaired to other heart diseases including congestive cardiomyopathy , hypertrophic obstrutive cardiomyopathy , myocarditis and sarcoidosis .
	manualset3
86149	3	398386	5	NULL	NULL	0	NULL	heart diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we demonstrate , that the overexpression of NCAM ( CD56 ) is specific for ischemic damage as compaired to other heart diseases including congestive cardiomyopathy , hypertrophic obstrutive cardiomyopathy , myocarditis and sarcoidosis .
	manualset3
86150	4	398386	5	NULL	NULL	0	NULL	congestive cardiomyopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we demonstrate , that the overexpression of NCAM ( CD56 ) is specific for ischemic damage as compaired to other heart diseases including congestive cardiomyopathy , hypertrophic obstrutive cardiomyopathy , myocarditis and sarcoidosis .
	manualset3
86151	5	398386	5	NULL	NULL	0	NULL	hypertrophic obstrutive cardiomyopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we demonstrate , that the overexpression of NCAM ( CD56 ) is specific for ischemic damage as compaired to other heart diseases including congestive cardiomyopathy , hypertrophic obstrutive cardiomyopathy , myocarditis and sarcoidosis .
	manualset3
86152	6	398386	5	NULL	NULL	0	NULL	myocarditis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we demonstrate , that the overexpression of NCAM ( CD56 ) is specific for ischemic damage as compaired to other heart diseases including congestive cardiomyopathy , hypertrophic obstrutive cardiomyopathy , myocarditis and sarcoidosis .
	manualset3
86153	7	398386	5	NULL	NULL	0	NULL	sarcoidosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we demonstrate , that the overexpression of NCAM ( CD56 ) is specific for ischemic damage as compaired to other heart diseases including congestive cardiomyopathy , hypertrophic obstrutive cardiomyopathy , myocarditis and sarcoidosis .
	manualset3
86154	1	398387	5	NULL	NULL	0	NULL	lipopeptides	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we demonstrate that lipopeptides also constitute adjuvants for mucosal immunizations .
	manualset3
86155	2	398387	5	NULL	NULL	0	NULL	adjuvants	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we demonstrate that lipopeptides also constitute adjuvants for mucosal immunizations .
	manualset3
86156	3	398387	5	NULL	NULL	0	NULL	mucosal immunizations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we demonstrate that lipopeptides also constitute adjuvants for mucosal immunizations .
	manualset3
86157	1	398388	5	NULL	NULL	0	NULL	LipA levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we demonstrate that the reduced LipA levels are due to the absence of four genes , skfABCD , located in the prophage 1 region .
	manualset3
86158	2	398388	5	NULL	NULL	NULL	NULL	four genes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we demonstrate that the reduced LipA levels are due to the absence of four genes , skfABCD , located in the prophage 1 region .
	manualset3
86159	3	398388	5	NULL	NULL	0	NULL	skfABCD	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we demonstrate that the reduced LipA levels are due to the absence of four genes , skfABCD , located in the prophage 1 region .
	manualset3
86160	4	398388	5	NULL	NULL	0	NULL	prophage 1 region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we demonstrate that the reduced LipA levels are due to the absence of four genes , skfABCD , located in the prophage 1 region .
	manualset3
86161	1	398389	5	NULL	NULL	0	NULL	p1-30	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we demonstrate the ability of p1-30 to act in synergy with IL-2 , -4 , -9 , and -15 .
	manualset3
86162	3	398389	5	NULL	NULL	NULL	NULL	IL-2 , -4 , -9 , and -15	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we demonstrate the ability of p1-30 to act in synergy with IL-2 , -4 , -9 , and -15 .
	manualset3
86489	2	398389	5	NULL	NULL	0	NULL	synergy 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we demonstrate the ability of p1-30 to act in synergy with IL-2 , -4 , -9 , and -15 .
	manualset3
86163	1	398390	5	NULL	NULL	0	NULL	CAP approach , called biotinylated CAP ( Bio-CAP )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe a new CAP approach , called biotinylated CAP ( Bio-CAP ) , which eliminates the requirement for specialized equipment while dramatically improving and simplifying the CxxC-based DNA affinity purification .
	manualset3
86164	2	398390	5	NULL	NULL	0	NULL	specialized equipment	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe a new CAP approach , called biotinylated CAP ( Bio-CAP ) , which eliminates the requirement for specialized equipment while dramatically improving and simplifying the CxxC-based DNA affinity purification .
	manualset3
86165	3	398390	5	NULL	NULL	0	NULL	CxxC-based DNA affinity purification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe a new CAP approach , called biotinylated CAP ( Bio-CAP ) , which eliminates the requirement for specialized equipment while dramatically improving and simplifying the CxxC-based DNA affinity purification .
	manualset3
86166	1	398391	5	NULL	NULL	0	NULL	novel database termed MaxQB	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe a novel database termed MaxQB that stores and displays collections of large proteomics projects and allows joint analysis and comparison .
	manualset3
86167	2	398391	5	NULL	NULL	0	NULL	large proteomics projects	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe a novel database termed MaxQB that stores and displays collections of large proteomics projects and allows joint analysis and comparison .
	manualset3
86168	3	398391	5	NULL	NULL	0	NULL	joint analysis and comparison	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe a novel database termed MaxQB that stores and displays collections of large proteomics projects and allows joint analysis and comparison .
	manualset3
86169	1	398392	5	NULL	NULL	0	NULL	DNA lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe a procedure to quantify DNA lesions recognized by the bacterial formamido-pyrimidine-DNA glycosylases ( Fpg protein ) .
	manualset3
86170	2	398392	5	NULL	NULL	0	NULL	bacterial formamido-pyrimidine-DNA glycosylases ( Fpg protein )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe a procedure to quantify DNA lesions recognized by the bacterial formamido-pyrimidine-DNA glycosylases ( Fpg protein ) .
	manualset3
86171	1	398393	5	NULL	NULL	0	NULL	Surgical treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Surgical treatment of myocardial infarct in complications .
	manualset3
86172	2	398393	5	NULL	NULL	0	NULL	myocardial infarct	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Surgical treatment of myocardial infarct in complications .
	manualset3
86173	3	398393	5	NULL	NULL	0	NULL	complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Surgical treatment of myocardial infarct in complications .
	manualset3
86174	1	398394	5	NULL	NULL	0	NULL	catalysis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe an advance in the catalysis of the overall splitting of water under visible light : the new catalyst is a solid solution of gallium and zinc nitrogen oxide , ( Ga ( 1-x ) Zn ( x ) ) ( N ( 1-x ) O ( x ) ) , modified with nanoparticles of a mixed oxide of rhodium and chromium .
	manualset3
86175	2	398394	5	NULL	NULL	0	NULL	splitting of water under visible light	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe an advance in the catalysis of the overall splitting of water under visible light : the new catalyst is a solid solution of gallium and zinc nitrogen oxide , ( Ga ( 1-x ) Zn ( x ) ) ( N ( 1-x ) O ( x ) ) , modified with nanoparticles of a mixed oxide of rhodium and chromium .
	manualset3
86176	3	398394	5	NULL	NULL	NULL	NULL	new catalyst	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we describe an advance in the catalysis of the overall splitting of water under visible light : the new catalyst is a solid solution of gallium and zinc nitrogen oxide , ( Ga ( 1-x ) Zn ( x ) ) ( N ( 1-x ) O ( x ) ) , modified with nanoparticles of a mixed oxide of rhodium and chromium .
	manualset3
86177	4	398394	5	NULL	NULL	NULL	NULL	solid solution of gallium and zinc nitrogen oxide , ( Ga ( 1-x ) Zn ( x ) ) ( N ( 1-x ) O ( x ) )	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we describe an advance in the catalysis of the overall splitting of water under visible light : the new catalyst is a solid solution of gallium and zinc nitrogen oxide , ( Ga ( 1-x ) Zn ( x ) ) ( N ( 1-x ) O ( x ) ) , modified with nanoparticles of a mixed oxide of rhodium and chromium .
	manualset3
86178	5	398394	5	NULL	NULL	NULL	NULL	nanoparticles of a mixed oxide of rhodium and chromium	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we describe an advance in the catalysis of the overall splitting of water under visible light : the new catalyst is a solid solution of gallium and zinc nitrogen oxide , ( Ga ( 1-x ) Zn ( x ) ) ( N ( 1-x ) O ( x ) ) , modified with nanoparticles of a mixed oxide of rhodium and chromium .
	manualset3
86341	1	398395	5	NULL	NULL	0	NULL	five stages	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe five stages of insular gyral and sulcal development closely related to gestational age : stage 1 : appearance of the first sulcus at 13-17 GWs , stage 2 : development of the periinsular sulci at 18-19 GWs , stage 3 : central sulci and opercularization of the insula at 20-22 GWs , stage 4 : covering of the posterior insula at 24-26 GWs , stage 5 : closure of the sylvian fissure at 27-28 GWs .
	manualset3
86342	2	398395	5	NULL	NULL	0	NULL	insular gyral and sulcal development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe five stages of insular gyral and sulcal development closely related to gestational age : stage 1 : appearance of the first sulcus at 13-17 GWs , stage 2 : development of the periinsular sulci at 18-19 GWs , stage 3 : central sulci and opercularization of the insula at 20-22 GWs , stage 4 : covering of the posterior insula at 24-26 GWs , stage 5 : closure of the sylvian fissure at 27-28 GWs .
	manualset3
86343	3	398395	5	NULL	NULL	0	NULL	gestational age	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe five stages of insular gyral and sulcal development closely related to gestational age : stage 1 : appearance of the first sulcus at 13-17 GWs , stage 2 : development of the periinsular sulci at 18-19 GWs , stage 3 : central sulci and opercularization of the insula at 20-22 GWs , stage 4 : covering of the posterior insula at 24-26 GWs , stage 5 : closure of the sylvian fissure at 27-28 GWs .
	manualset3
86344	4	398395	5	NULL	NULL	0	NULL	stage 1	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe five stages of insular gyral and sulcal development closely related to gestational age : stage 1 : appearance of the first sulcus at 13-17 GWs , stage 2 : development of the periinsular sulci at 18-19 GWs , stage 3 : central sulci and opercularization of the insula at 20-22 GWs , stage 4 : covering of the posterior insula at 24-26 GWs , stage 5 : closure of the sylvian fissure at 27-28 GWs .
	manualset3
86345	5	398395	5	NULL	NULL	0	NULL	appearance of the first sulcus at 13-17 GWs	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe five stages of insular gyral and sulcal development closely related to gestational age : stage 1 : appearance of the first sulcus at 13-17 GWs , stage 2 : development of the periinsular sulci at 18-19 GWs , stage 3 : central sulci and opercularization of the insula at 20-22 GWs , stage 4 : covering of the posterior insula at 24-26 GWs , stage 5 : closure of the sylvian fissure at 27-28 GWs .
	manualset3
86346	6	398395	5	NULL	NULL	0	NULL	stage 2	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe five stages of insular gyral and sulcal development closely related to gestational age : stage 1 : appearance of the first sulcus at 13-17 GWs , stage 2 : development of the periinsular sulci at 18-19 GWs , stage 3 : central sulci and opercularization of the insula at 20-22 GWs , stage 4 : covering of the posterior insula at 24-26 GWs , stage 5 : closure of the sylvian fissure at 27-28 GWs .
	manualset3
86347	7	398395	5	NULL	NULL	0	NULL	development of the periinsular sulci at 18-19 GWs	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe five stages of insular gyral and sulcal development closely related to gestational age : stage 1 : appearance of the first sulcus at 13-17 GWs , stage 2 : development of the periinsular sulci at 18-19 GWs , stage 3 : central sulci and opercularization of the insula at 20-22 GWs , stage 4 : covering of the posterior insula at 24-26 GWs , stage 5 : closure of the sylvian fissure at 27-28 GWs .
	manualset3
86348	8	398395	5	NULL	NULL	0	NULL	stage 3	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe five stages of insular gyral and sulcal development closely related to gestational age : stage 1 : appearance of the first sulcus at 13-17 GWs , stage 2 : development of the periinsular sulci at 18-19 GWs , stage 3 : central sulci and opercularization of the insula at 20-22 GWs , stage 4 : covering of the posterior insula at 24-26 GWs , stage 5 : closure of the sylvian fissure at 27-28 GWs .
	manualset3
86349	9	398395	5	NULL	NULL	0	NULL	central sulci and opercularization of the insula at 20-22 GWs	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe five stages of insular gyral and sulcal development closely related to gestational age : stage 1 : appearance of the first sulcus at 13-17 GWs , stage 2 : development of the periinsular sulci at 18-19 GWs , stage 3 : central sulci and opercularization of the insula at 20-22 GWs , stage 4 : covering of the posterior insula at 24-26 GWs , stage 5 : closure of the sylvian fissure at 27-28 GWs .
	manualset3
86350	10	398395	5	NULL	NULL	0	NULL	stage 4	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe five stages of insular gyral and sulcal development closely related to gestational age : stage 1 : appearance of the first sulcus at 13-17 GWs , stage 2 : development of the periinsular sulci at 18-19 GWs , stage 3 : central sulci and opercularization of the insula at 20-22 GWs , stage 4 : covering of the posterior insula at 24-26 GWs , stage 5 : closure of the sylvian fissure at 27-28 GWs .
	manualset3
86351	11	398395	5	NULL	NULL	0	NULL	covering of the posterior insula at 24-26 GWs	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe five stages of insular gyral and sulcal development closely related to gestational age : stage 1 : appearance of the first sulcus at 13-17 GWs , stage 2 : development of the periinsular sulci at 18-19 GWs , stage 3 : central sulci and opercularization of the insula at 20-22 GWs , stage 4 : covering of the posterior insula at 24-26 GWs , stage 5 : closure of the sylvian fissure at 27-28 GWs .
	manualset3
86352	12	398395	5	NULL	NULL	0	NULL	stage 5	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe five stages of insular gyral and sulcal development closely related to gestational age : stage 1 : appearance of the first sulcus at 13-17 GWs , stage 2 : development of the periinsular sulci at 18-19 GWs , stage 3 : central sulci and opercularization of the insula at 20-22 GWs , stage 4 : covering of the posterior insula at 24-26 GWs , stage 5 : closure of the sylvian fissure at 27-28 GWs .
	manualset3
86353	13	398395	5	NULL	NULL	0	NULL	closure of the sylvian fissure at 27-28 GWs	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe five stages of insular gyral and sulcal development closely related to gestational age : stage 1 : appearance of the first sulcus at 13-17 GWs , stage 2 : development of the periinsular sulci at 18-19 GWs , stage 3 : central sulci and opercularization of the insula at 20-22 GWs , stage 4 : covering of the posterior insula at 24-26 GWs , stage 5 : closure of the sylvian fissure at 27-28 GWs .
	manualset3
86179	1	398396	5	NULL	NULL	NULL	NULL	mass precision	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we describe how mass precision for each peptide increases successively by considering all associated measurements , starting from the MS peak and proceeding to its chromatographic elution profile , isotope envelope , and stable isotope pair in SILAC measurements .
	manualset3
86180	2	398396	5	NULL	NULL	0	NULL	peptide	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe how mass precision for each peptide increases successively by considering all associated measurements , starting from the MS peak and proceeding to its chromatographic elution profile , isotope envelope , and stable isotope pair in SILAC measurements .
	manualset3
86181	3	398396	5	NULL	NULL	NULL	NULL	MS peak	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we describe how mass precision for each peptide increases successively by considering all associated measurements , starting from the MS peak and proceeding to its chromatographic elution profile , isotope envelope , and stable isotope pair in SILAC measurements .
	manualset3
86182	4	398396	5	NULL	NULL	NULL	NULL	chromatographic elution profile	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we describe how mass precision for each peptide increases successively by considering all associated measurements , starting from the MS peak and proceeding to its chromatographic elution profile , isotope envelope , and stable isotope pair in SILAC measurements .
	manualset3
86183	5	398396	5	NULL	NULL	NULL	NULL	isotope envelope	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we describe how mass precision for each peptide increases successively by considering all associated measurements , starting from the MS peak and proceeding to its chromatographic elution profile , isotope envelope , and stable isotope pair in SILAC measurements .
	manualset3
86184	6	398396	5	NULL	NULL	NULL	NULL	stable isotope pair in SILAC measurements	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we describe how mass precision for each peptide increases successively by considering all associated measurements , starting from the MS peak and proceeding to its chromatographic elution profile , isotope envelope , and stable isotope pair in SILAC measurements .
	manualset3
86185	1	398397	5	NULL	NULL	0	NULL	young male	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe the case of young male with , long-standing progressive vitiligo , presenting with congestive cardiac failure due to dilated cardiomyopathy and primary hypothyroidism .
	manualset3
86186	2	398397	5	NULL	NULL	0	NULL	 long-standing progressive vitiligo	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe the case of young male with , long-standing progressive vitiligo , presenting with congestive cardiac failure due to dilated cardiomyopathy and primary hypothyroidism .
	manualset3
86187	3	398397	5	NULL	NULL	0	NULL	congestive cardiac failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe the case of young male with , long-standing progressive vitiligo , presenting with congestive cardiac failure due to dilated cardiomyopathy and primary hypothyroidism .
	manualset3
86188	4	398397	5	NULL	NULL	0	NULL	dilated cardiomyopathy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe the case of young male with , long-standing progressive vitiligo , presenting with congestive cardiac failure due to dilated cardiomyopathy and primary hypothyroidism .
	manualset3
86189	5	398397	5	NULL	NULL	0	NULL	primary hypothyroidism	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe the case of young male with , long-standing progressive vitiligo , presenting with congestive cardiac failure due to dilated cardiomyopathy and primary hypothyroidism .
	manualset3
86190	1	398398	5	NULL	NULL	NULL	NULL	cryptic chromosomally encoded 34-kDa cytolysin A hemolysin of Salmonella enterica serovar Typhi ( ClyA )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we describe the cryptic chromosomally encoded 34-kDa cytolysin A hemolysin of Salmonella enterica serovar Typhi ( ClyA ) as a novel export system for the expression of heterologous antigens in the supernatant of attenuated Salmonella serovar Typhi live-vector vaccine strains .
	manualset3
86191	2	398398	5	NULL	NULL	0	NULL	novel export system	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe the cryptic chromosomally encoded 34-kDa cytolysin A hemolysin of Salmonella enterica serovar Typhi ( ClyA ) as a novel export system for the expression of heterologous antigens in the supernatant of attenuated Salmonella serovar Typhi live-vector vaccine strains .
	manualset3
86192	3	398398	5	NULL	NULL	0	NULL	expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe the cryptic chromosomally encoded 34-kDa cytolysin A hemolysin of Salmonella enterica serovar Typhi ( ClyA ) as a novel export system for the expression of heterologous antigens in the supernatant of attenuated Salmonella serovar Typhi live-vector vaccine strains .
	manualset3
86193	4	398398	5	NULL	NULL	0	NULL	heterologous antigens	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe the cryptic chromosomally encoded 34-kDa cytolysin A hemolysin of Salmonella enterica serovar Typhi ( ClyA ) as a novel export system for the expression of heterologous antigens in the supernatant of attenuated Salmonella serovar Typhi live-vector vaccine strains .
	manualset3
86194	5	398398	5	NULL	NULL	0	NULL	attenuated Salmonella serovar Typhi live-vector vaccine strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe the cryptic chromosomally encoded 34-kDa cytolysin A hemolysin of Salmonella enterica serovar Typhi ( ClyA ) as a novel export system for the expression of heterologous antigens in the supernatant of attenuated Salmonella serovar Typhi live-vector vaccine strains .
	manualset3
86195	1	398399	5	NULL	NULL	0	NULL	expression pattern of HTm4	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe the expression pattern of HTm4 in peripheral blood cells using gene expression microarray technology , and in normal foetal and adult human tissues , as well as adult human cancers , using tissue microarray technology .
	manualset3
86196	2	398399	5	NULL	NULL	0	NULL	peripheral blood cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe the expression pattern of HTm4 in peripheral blood cells using gene expression microarray technology , and in normal foetal and adult human tissues , as well as adult human cancers , using tissue microarray technology .
	manualset3
86197	3	398399	5	NULL	NULL	0	NULL	gene expression microarray technology	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe the expression pattern of HTm4 in peripheral blood cells using gene expression microarray technology , and in normal foetal and adult human tissues , as well as adult human cancers , using tissue microarray technology .
	manualset3
86198	4	398399	5	NULL	NULL	0	NULL	normal foetal and adult human tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe the expression pattern of HTm4 in peripheral blood cells using gene expression microarray technology , and in normal foetal and adult human tissues , as well as adult human cancers , using tissue microarray technology .
	manualset3
86199	5	398399	5	NULL	NULL	0	NULL	adult human cancers	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe the expression pattern of HTm4 in peripheral blood cells using gene expression microarray technology , and in normal foetal and adult human tissues , as well as adult human cancers , using tissue microarray technology .
	manualset3
86200	6	398399	5	NULL	NULL	0	NULL	tissue microarray technology	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we describe the expression pattern of HTm4 in peripheral blood cells using gene expression microarray technology , and in normal foetal and adult human tissues , as well as adult human cancers , using tissue microarray technology .
	manualset3
86201	1	398400	5	NULL	NULL	0	NULL	de novo spine formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we develop an approach to induce and monitor de novo spine formation in real time using combined two-photon laser-scanning microscopy and two-photon laser uncaging of glutamate .
	manualset3
86202	2	398400	5	NULL	NULL	0	NULL	real time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we develop an approach to induce and monitor de novo spine formation in real time using combined two-photon laser-scanning microscopy and two-photon laser uncaging of glutamate .
	manualset3
86203	3	398400	5	NULL	NULL	NULL	NULL	two-photon laser-scanning microscopy	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we develop an approach to induce and monitor de novo spine formation in real time using combined two-photon laser-scanning microscopy and two-photon laser uncaging of glutamate .
	manualset3
86493	4	398400	5	NULL	NULL	0	NULL	two-photon laser uncaging of glutamate	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we develop an approach to induce and monitor de novo spine formation in real time using combined two-photon laser-scanning microscopy and two-photon laser uncaging of glutamate .
	manualset3
86204	1	398401	5	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we disclose studies examining the use of large amplitude voltage excitations ( applied for short periods of time ) to cause fragmentation of the ions of interest .
	manualset3
86205	2	398401	5	NULL	NULL	0	NULL	large amplitude voltage excitations	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we disclose studies examining the use of large amplitude voltage excitations ( applied for short periods of time ) to cause fragmentation of the ions of interest .
	manualset3
86206	3	398401	5	NULL	NULL	0	NULL	short periods of time	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we disclose studies examining the use of large amplitude voltage excitations ( applied for short periods of time ) to cause fragmentation of the ions of interest .
	manualset3
86207	4	398401	5	NULL	NULL	0	NULL	fragmentation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we disclose studies examining the use of large amplitude voltage excitations ( applied for short periods of time ) to cause fragmentation of the ions of interest .
	manualset3
86208	5	398401	5	NULL	NULL	0	NULL	ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we disclose studies examining the use of large amplitude voltage excitations ( applied for short periods of time ) to cause fragmentation of the ions of interest .
	manualset3
86209	1	398402	5	NULL	NULL	0	NULL	mechanisms of RUNX3	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we discuss recent breakthroughs in our understanding of the mechanisms of RUNX3 in gastric malignancy and comment on possible future trends and perspectives .
	manualset3
86210	2	398402	5	NULL	NULL	0	NULL	gastric malignancy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we discuss recent breakthroughs in our understanding of the mechanisms of RUNX3 in gastric malignancy and comment on possible future trends and perspectives .
	manualset3
87583	3	398402	5	NULL	NULL	0	NULL	breakthroughs in our understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we discuss recent breakthroughs in our understanding of the mechanisms of RUNX3 in gastric malignancy and comment on possible future trends and perspectives .
	manualset3
86211	1	398403	5	NULL	NULL	0	NULL	distribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine the distribution of cannabinoid receptors and endocannabinoid-hydrolyzing enzymes within pain modulatory circuits together with behavioral , neurochemical , and neurophysiological studies that suggest a role for endocannabinoid signaling in pain modulation .
	manualset3
86212	2	398403	5	NULL	NULL	0	NULL	cannabinoid receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine the distribution of cannabinoid receptors and endocannabinoid-hydrolyzing enzymes within pain modulatory circuits together with behavioral , neurochemical , and neurophysiological studies that suggest a role for endocannabinoid signaling in pain modulation .
	manualset3
86213	3	398403	5	NULL	NULL	0	NULL	endocannabinoid-hydrolyzing enzymes	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine the distribution of cannabinoid receptors and endocannabinoid-hydrolyzing enzymes within pain modulatory circuits together with behavioral , neurochemical , and neurophysiological studies that suggest a role for endocannabinoid signaling in pain modulation .
	manualset3
86214	4	398403	5	NULL	NULL	0	NULL	 pain modulatory circuits	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine the distribution of cannabinoid receptors and endocannabinoid-hydrolyzing enzymes within pain modulatory circuits together with behavioral , neurochemical , and neurophysiological studies that suggest a role for endocannabinoid signaling in pain modulation .
	manualset3
86215	5	398403	5	NULL	NULL	0	NULL	behavioral studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine the distribution of cannabinoid receptors and endocannabinoid-hydrolyzing enzymes within pain modulatory circuits together with behavioral , neurochemical , and neurophysiological studies that suggest a role for endocannabinoid signaling in pain modulation .
	manualset3
86216	6	398403	5	NULL	NULL	0	NULL	neurochemical studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine the distribution of cannabinoid receptors and endocannabinoid-hydrolyzing enzymes within pain modulatory circuits together with behavioral , neurochemical , and neurophysiological studies that suggest a role for endocannabinoid signaling in pain modulation .
	manualset3
86217	7	398403	5	NULL	NULL	0	NULL	neurophysiological studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine the distribution of cannabinoid receptors and endocannabinoid-hydrolyzing enzymes within pain modulatory circuits together with behavioral , neurochemical , and neurophysiological studies that suggest a role for endocannabinoid signaling in pain modulation .
	manualset3
86218	8	398403	5	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine the distribution of cannabinoid receptors and endocannabinoid-hydrolyzing enzymes within pain modulatory circuits together with behavioral , neurochemical , and neurophysiological studies that suggest a role for endocannabinoid signaling in pain modulation .
	manualset3
86219	9	398403	5	NULL	NULL	0	NULL	endocannabinoid signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine the distribution of cannabinoid receptors and endocannabinoid-hydrolyzing enzymes within pain modulatory circuits together with behavioral , neurochemical , and neurophysiological studies that suggest a role for endocannabinoid signaling in pain modulation .
	manualset3
86220	10	398403	5	NULL	NULL	0	NULL	pain modulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine the distribution of cannabinoid receptors and endocannabinoid-hydrolyzing enzymes within pain modulatory circuits together with behavioral , neurochemical , and neurophysiological studies that suggest a role for endocannabinoid signaling in pain modulation .
	manualset3
86221	1	398404	5	NULL	NULL	0	NULL	partner preference formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine the effects on partner preference formation in male prairie voles of neurochemical manipulations in the ventral tegmental area ( VTA ) , a major source of dopamine to brain regions implicated in pair bonding .
	manualset3
86222	2	398404	5	NULL	NULL	0	NULL	male prairie voles	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine the effects on partner preference formation in male prairie voles of neurochemical manipulations in the ventral tegmental area ( VTA ) , a major source of dopamine to brain regions implicated in pair bonding .
	manualset3
86223	3	398404	5	NULL	NULL	0	NULL	neurochemical manipulations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine the effects on partner preference formation in male prairie voles of neurochemical manipulations in the ventral tegmental area ( VTA ) , a major source of dopamine to brain regions implicated in pair bonding .
	manualset3
86224	4	398404	5	NULL	NULL	0	NULL	ventral tegmental area ( VTA )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine the effects on partner preference formation in male prairie voles of neurochemical manipulations in the ventral tegmental area ( VTA ) , a major source of dopamine to brain regions implicated in pair bonding .
	manualset3
86225	5	398404	5	NULL	NULL	0	NULL	dopamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine the effects on partner preference formation in male prairie voles of neurochemical manipulations in the ventral tegmental area ( VTA ) , a major source of dopamine to brain regions implicated in pair bonding .
	manualset3
86226	6	398404	5	NULL	NULL	0	NULL	brain regions implicated in pair bonding	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine the effects on partner preference formation in male prairie voles of neurochemical manipulations in the ventral tegmental area ( VTA ) , a major source of dopamine to brain regions implicated in pair bonding .
	manualset3
86227	1	398405	5	NULL	NULL	0	NULL	stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine their stimulation of antigen-specific CD4 ( + ) T cells , critical for protective immunity against tumors or infectious disease .
	manualset3
86228	2	398405	5	NULL	NULL	0	NULL	antigen-specific CD4 ( + ) T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine their stimulation of antigen-specific CD4 ( + ) T cells , critical for protective immunity against tumors or infectious disease .
	manualset3
86229	3	398405	5	NULL	NULL	0	NULL	protective immunity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine their stimulation of antigen-specific CD4 ( + ) T cells , critical for protective immunity against tumors or infectious disease .
	manualset3
86230	4	398405	5	NULL	NULL	0	NULL	tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine their stimulation of antigen-specific CD4 ( + ) T cells , critical for protective immunity against tumors or infectious disease .
	manualset3
86231	5	398405	5	NULL	NULL	0	NULL	infectious disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine their stimulation of antigen-specific CD4 ( + ) T cells , critical for protective immunity against tumors or infectious disease .
	manualset3
86232	1	398406	5	NULL	NULL	0	NULL	captopril , an angiotensin converting enzyme inhibitor	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examined effects of captopril , an angiotensin converting enzyme inhibitor , on serum lipid levels and oxygen consumption rate in mitochondria isolated from heart of rabbits treated by hypercholesterolemic diet .
	manualset3
86233	2	398406	5	NULL	NULL	0	NULL	serum lipid levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examined effects of captopril , an angiotensin converting enzyme inhibitor , on serum lipid levels and oxygen consumption rate in mitochondria isolated from heart of rabbits treated by hypercholesterolemic diet .
	manualset3
86234	3	398406	5	NULL	NULL	0	NULL	oxygen consumption rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examined effects of captopril , an angiotensin converting enzyme inhibitor , on serum lipid levels and oxygen consumption rate in mitochondria isolated from heart of rabbits treated by hypercholesterolemic diet .
	manualset3
86235	4	398406	5	NULL	NULL	0	NULL	mitochondria	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examined effects of captopril , an angiotensin converting enzyme inhibitor , on serum lipid levels and oxygen consumption rate in mitochondria isolated from heart of rabbits treated by hypercholesterolemic diet .
	manualset3
86236	5	398406	5	NULL	NULL	0	NULL	heart 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examined effects of captopril , an angiotensin converting enzyme inhibitor , on serum lipid levels and oxygen consumption rate in mitochondria isolated from heart of rabbits treated by hypercholesterolemic diet .
	manualset3
86237	6	398406	5	NULL	NULL	0	NULL	rabbits	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examined effects of captopril , an angiotensin converting enzyme inhibitor , on serum lipid levels and oxygen consumption rate in mitochondria isolated from heart of rabbits treated by hypercholesterolemic diet .
	manualset3
86238	7	398406	5	NULL	NULL	0	NULL	hypercholesterolemic diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examined effects of captopril , an angiotensin converting enzyme inhibitor , on serum lipid levels and oxygen consumption rate in mitochondria isolated from heart of rabbits treated by hypercholesterolemic diet .
	manualset3
86239	1	398407	5	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we explored the role of CD8 ( + ) T-cells in T. cruzi-elicited heart injury in C57BL/6 mice infected with the Colombian strain .
	manualset3
86240	2	398407	5	NULL	NULL	0	NULL	CD8 ( + ) T-cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we explored the role of CD8 ( + ) T-cells in T. cruzi-elicited heart injury in C57BL/6 mice infected with the Colombian strain .
	manualset3
86241	3	398407	5	NULL	NULL	0	NULL	T. cruzi-elicited heart injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we explored the role of CD8 ( + ) T-cells in T. cruzi-elicited heart injury in C57BL/6 mice infected with the Colombian strain .
	manualset3
86242	4	398407	5	NULL	NULL	0	NULL	C57BL/6 mice infected with the Colombian strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we explored the role of CD8 ( + ) T-cells in T. cruzi-elicited heart injury in C57BL/6 mice infected with the Colombian strain .
	manualset3
86243	1	398408	5	NULL	NULL	0	NULL	influenza virus reporter cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we generated an influenza virus reporter cell line in which the luciferase gene was driven by the influenza virus promoter and screened a small compound library ( NCI Diversity Set II ) .
	manualset3
86244	2	398408	5	NULL	NULL	0	NULL	luciferase gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we generated an influenza virus reporter cell line in which the luciferase gene was driven by the influenza virus promoter and screened a small compound library ( NCI Diversity Set II ) .
	manualset3
86245	3	398408	5	NULL	NULL	0	NULL	influenza virus promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we generated an influenza virus reporter cell line in which the luciferase gene was driven by the influenza virus promoter and screened a small compound library ( NCI Diversity Set II ) .
	manualset3
86246	4	398408	5	NULL	NULL	0	NULL	small compound library ( NCI Diversity Set II )	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we generated an influenza virus reporter cell line in which the luciferase gene was driven by the influenza virus promoter and screened a small compound library ( NCI Diversity Set II ) .
	manualset3
86247	1	398409	5	NULL	NULL	0	NULL	FLAG-fused Orai1 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we have purified the FLAG-fused Orai1 protein , determined its tetrameric stoichiometry , and reconstructed its three-dimensional structure at 21-A resolution from 3681 automatically selected particle images , taken with an electron microscope .
	manualset3
86248	2	398409	5	NULL	NULL	0	NULL	tetrameric stoichiometry	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we have purified the FLAG-fused Orai1 protein , determined its tetrameric stoichiometry , and reconstructed its three-dimensional structure at 21-A resolution from 3681 automatically selected particle images , taken with an electron microscope .
	manualset3
86249	3	398409	5	NULL	NULL	0	NULL	three-dimensional structure	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we have purified the FLAG-fused Orai1 protein , determined its tetrameric stoichiometry , and reconstructed its three-dimensional structure at 21-A resolution from 3681 automatically selected particle images , taken with an electron microscope .
	manualset3
86250	4	398409	5	NULL	NULL	0	NULL	21-A resolution	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we have purified the FLAG-fused Orai1 protein , determined its tetrameric stoichiometry , and reconstructed its three-dimensional structure at 21-A resolution from 3681 automatically selected particle images , taken with an electron microscope .
	manualset3
86251	5	398409	5	NULL	NULL	0	NULL	3681 automatically selected particle images	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we have purified the FLAG-fused Orai1 protein , determined its tetrameric stoichiometry , and reconstructed its three-dimensional structure at 21-A resolution from 3681 automatically selected particle images , taken with an electron microscope .
	manualset3
86252	6	398409	5	NULL	NULL	0	NULL	electron microscope	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we have purified the FLAG-fused Orai1 protein , determined its tetrameric stoichiometry , and reconstructed its three-dimensional structure at 21-A resolution from 3681 automatically selected particle images , taken with an electron microscope .
	manualset3
86253	1	398410	5	NULL	NULL	0	NULL	Survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Survival of intestinal bacilli in oil-polluted sea water ) .
	manualset3
86254	2	398410	5	NULL	NULL	0	NULL	intestinal bacilli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Survival of intestinal bacilli in oil-polluted sea water ) .
	manualset3
86255	3	398410	5	NULL	NULL	0	NULL	oil-polluted sea water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Survival of intestinal bacilli in oil-polluted sea water ) .
	manualset3
86256	1	398411	5	NULL	NULL	0	NULL	novel mass spectrometry-based imaging technique called cation-enhanced nanostructure-initiator mass spectrometry ( NIMS )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we have used a novel mass spectrometry-based imaging technique called cation-enhanced nanostructure-initiator mass spectrometry ( NIMS ) for the in situ detection of intact cholesterol molecules from biological tissues .
	manualset3
86257	3	398411	5	NULL	NULL	NULL	NULL	intact cholesterol molecules	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we have used a novel mass spectrometry-based imaging technique called cation-enhanced nanostructure-initiator mass spectrometry ( NIMS ) for the in situ detection of intact cholesterol molecules from biological tissues .
	manualset3
86258	3	398411	5	NULL	NULL	0	NULL	biological tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we have used a novel mass spectrometry-based imaging technique called cation-enhanced nanostructure-initiator mass spectrometry ( NIMS ) for the in situ detection of intact cholesterol molecules from biological tissues .
	manualset3
87584	2	398411	5	NULL	NULL	0	NULL	in situ detection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we have used a novel mass spectrometry-based imaging technique called cation-enhanced nanostructure-initiator mass spectrometry ( NIMS ) for the in situ detection of intact cholesterol molecules from biological tissues .
	manualset3
86259	1	398412	5	NULL	NULL	0	NULL	LXR activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we investigated the influence of LXR activation on intracellular cholesterol trafficking in primary human macrophages .
	manualset3
86260	2	398412	5	NULL	NULL	0	NULL	intracellular cholesterol trafficking	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we investigated the influence of LXR activation on intracellular cholesterol trafficking in primary human macrophages .
	manualset3
86261	3	398412	5	NULL	NULL	0	NULL	primary human macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we investigated the influence of LXR activation on intracellular cholesterol trafficking in primary human macrophages .
	manualset3
86262	1	398413	5	NULL	NULL	0	NULL	receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we investigated the presence and characteristics of such receptors in the rat LSO by means of whole-cell patch-clamp recordings in combination with pharmacology .
	manualset3
86263	2	398413	5	NULL	NULL	0	NULL	rat LSO	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we investigated the presence and characteristics of such receptors in the rat LSO by means of whole-cell patch-clamp recordings in combination with pharmacology .
	manualset3
86264	3	398413	5	NULL	NULL	0	NULL	whole-cell patch-clamp recordings	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we investigated the presence and characteristics of such receptors in the rat LSO by means of whole-cell patch-clamp recordings in combination with pharmacology .
	manualset3
86265	4	398413	5	NULL	NULL	0	NULL	pharmacology	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we investigated the presence and characteristics of such receptors in the rat LSO by means of whole-cell patch-clamp recordings in combination with pharmacology .
	manualset3
86266	1	398414	5	NULL	NULL	0	NULL	time constants	Unit												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we note that the time constants involved in this latter type of field sensitivity are much longer than those in organisms that make use of the earth 's magnetic field for navigation .
	manualset3
86267	2	398414	5	NULL	NULL	0	NULL	field sensitivity	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we note that the time constants involved in this latter type of field sensitivity are much longer than those in organisms that make use of the earth 's magnetic field for navigation .
	manualset3
86268	3	398414	5	NULL	NULL	0	NULL	organisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we note that the time constants involved in this latter type of field sensitivity are much longer than those in organisms that make use of the earth 's magnetic field for navigation .
	manualset3
86269	4	398414	5	NULL	NULL	0	NULL	earth 's magnetic field	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we note that the time constants involved in this latter type of field sensitivity are much longer than those in organisms that make use of the earth 's magnetic field for navigation .
	manualset3
86270	5	398414	5	NULL	NULL	0	NULL	navigation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we note that the time constants involved in this latter type of field sensitivity are much longer than those in organisms that make use of the earth 's magnetic field for navigation .
	manualset3
86271	1	398415	5	NULL	NULL	0	NULL	whole-cell patch-clamp recordings	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we performed whole-cell patch clamp recordings from CA1 stratum radiatum interneurons in rat brain slices to investigate the effect of the eCB anandamide on excitatory synapses as well as the involvement of Group I metabotropic glutamate receptors ( mGluRs ) , which have been reported to produce eCBs endogenously .
	manualset3
86272	2	398415	5	NULL	NULL	0	NULL	CA1 stratum radiatum interneurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we performed whole-cell patch clamp recordings from CA1 stratum radiatum interneurons in rat brain slices to investigate the effect of the eCB anandamide on excitatory synapses as well as the involvement of Group I metabotropic glutamate receptors ( mGluRs ) , which have been reported to produce eCBs endogenously .
	manualset3
86273	3	398415	5	NULL	NULL	0	NULL	rat brain slices	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we performed whole-cell patch clamp recordings from CA1 stratum radiatum interneurons in rat brain slices to investigate the effect of the eCB anandamide on excitatory synapses as well as the involvement of Group I metabotropic glutamate receptors ( mGluRs ) , which have been reported to produce eCBs endogenously .
	manualset3
86274	4	398415	5	NULL	NULL	NULL	NULL	eCB anandamide	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we performed whole-cell patch clamp recordings from CA1 stratum radiatum interneurons in rat brain slices to investigate the effect of the eCB anandamide on excitatory synapses as well as the involvement of Group I metabotropic glutamate receptors ( mGluRs ) , which have been reported to produce eCBs endogenously .
	manualset3
86275	5	398415	5	NULL	NULL	0	NULL	excitatory synapses	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we performed whole-cell patch clamp recordings from CA1 stratum radiatum interneurons in rat brain slices to investigate the effect of the eCB anandamide on excitatory synapses as well as the involvement of Group I metabotropic glutamate receptors ( mGluRs ) , which have been reported to produce eCBs endogenously .
	manualset3
86276	6	398415	5	NULL	NULL	0	NULL	Group I metabotropic glutamate receptors ( mGluRs )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we performed whole-cell patch clamp recordings from CA1 stratum radiatum interneurons in rat brain slices to investigate the effect of the eCB anandamide on excitatory synapses as well as the involvement of Group I metabotropic glutamate receptors ( mGluRs ) , which have been reported to produce eCBs endogenously .
	manualset3
86277	7	398415	5	NULL	NULL	0	NULL	eCBs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we performed whole-cell patch clamp recordings from CA1 stratum radiatum interneurons in rat brain slices to investigate the effect of the eCB anandamide on excitatory synapses as well as the involvement of Group I metabotropic glutamate receptors ( mGluRs ) , which have been reported to produce eCBs endogenously .
	manualset3
86278	1	398416	5	NULL	NULL	NULL	NULL	PEM case	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we present a PEM case with R1150W polymorphism in SCN9A and a five-year remission was achieved by chemical lumbar sympathectomy ( CLS ) .
	manualset3
86279	2	398416	5	NULL	NULL	0	NULL	R1150W polymorphism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we present a PEM case with R1150W polymorphism in SCN9A and a five-year remission was achieved by chemical lumbar sympathectomy ( CLS ) .
	manualset3
86280	3	398416	5	NULL	NULL	0	NULL	SCN9A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we present a PEM case with R1150W polymorphism in SCN9A and a five-year remission was achieved by chemical lumbar sympathectomy ( CLS ) .
	manualset3
86281	4	398416	5	NULL	NULL	0	NULL	five-year remission	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we present a PEM case with R1150W polymorphism in SCN9A and a five-year remission was achieved by chemical lumbar sympathectomy ( CLS ) .
	manualset3
86282	5	398416	5	NULL	NULL	0	NULL	chemical lumbar sympathectomy ( CLS )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we present a PEM case with R1150W polymorphism in SCN9A and a five-year remission was achieved by chemical lumbar sympathectomy ( CLS ) .
	manualset3
86283	1	398417	5	NULL	NULL	0	NULL	theoretical argument	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we present a theoretical argument that motion differences can account for the direction of bias seen in humans .
	manualset3
86284	2	398417	5	NULL	NULL	0	NULL	motion differences	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we present a theoretical argument that motion differences can account for the direction of bias seen in humans .
	manualset3
86285	3	398417	5	NULL	NULL	0	NULL	bias	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we present a theoretical argument that motion differences can account for the direction of bias seen in humans .
	manualset3
86286	4	398417	5	NULL	NULL	0	NULL	humans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we present a theoretical argument that motion differences can account for the direction of bias seen in humans .
	manualset3
86287	1	398418	5	NULL	NULL	0	NULL	behavioral data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we present behavioral data and experiments from within nests of an ambrosia beetle , Xyleborinus saxesenii .
	manualset3
86288	2	398418	5	NULL	NULL	0	NULL	experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we present behavioral data and experiments from within nests of an ambrosia beetle , Xyleborinus saxesenii .
	manualset3
86289	3	398418	5	NULL	NULL	0	NULL	nests	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we present behavioral data and experiments from within nests of an ambrosia beetle , Xyleborinus saxesenii .
	manualset3
86290	4	398418	5	NULL	NULL	0	NULL	ambrosia beetle , Xyleborinus saxesenii	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we present behavioral data and experiments from within nests of an ambrosia beetle , Xyleborinus saxesenii .
	manualset3
86291	1	398419	5	NULL	NULL	0	NULL	Anaerobic organisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Anaerobic organisms , bacteremia and septicemia ) .
	manualset3
86292	2	398419	5	NULL	NULL	0	NULL	bacteremia	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Anaerobic organisms , bacteremia and septicemia ) .
	manualset3
86293	3	398419	5	NULL	NULL	0	NULL	septicemia	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Anaerobic organisms , bacteremia and septicemia ) .
	manualset3
86294	1	398420	5	NULL	NULL	0	NULL	Surviving case	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( Surviving case of Legionella pneumonia showing a high level of serum KL-6 and complicated with rhabdomyolysis ) .
	manualset3
86295	2	398420	5	NULL	NULL	0	NULL	Legionella pneumonia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Surviving case of Legionella pneumonia showing a high level of serum KL-6 and complicated with rhabdomyolysis ) .
	manualset3
86296	3	398420	5	NULL	NULL	0	NULL	high level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Surviving case of Legionella pneumonia showing a high level of serum KL-6 and complicated with rhabdomyolysis ) .
	manualset3
86297	4	398420	5	NULL	NULL	0	NULL	serum KL-6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Surviving case of Legionella pneumonia showing a high level of serum KL-6 and complicated with rhabdomyolysis ) .
	manualset3
86298	5	398420	5	NULL	NULL	0	NULL	rhabdomyolysis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Surviving case of Legionella pneumonia showing a high level of serum KL-6 and complicated with rhabdomyolysis ) .
	manualset3
86299	1	398421	5	NULL	NULL	NULL	NULL	location of a second prostate cancer susceptibility gene	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we present evidence for the location of a second prostate cancer susceptibility gene , which by heterogeneity estimates accounts for approximately 16 % of HPC cases .
	manualset3
86300	2	398421	5	NULL	NULL	0	NULL	heterogeneity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we present evidence for the location of a second prostate cancer susceptibility gene , which by heterogeneity estimates accounts for approximately 16 % of HPC cases .
	manualset3
86301	3	398421	5	NULL	NULL	0	NULL	16 % of HPC cases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we present evidence for the location of a second prostate cancer susceptibility gene , which by heterogeneity estimates accounts for approximately 16 % of HPC cases .
	manualset3
86302	1	398422	5	NULL	NULL	0	NULL	seven co-crystal structures of PDE4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we present seven co-crystal structures of PDE4 and bound inhibitors that show the regulatory domain closed across the active site , thereby revealing the structural basis of PDE4 regulation .
	manualset3
86303	2	398422	5	NULL	NULL	0	NULL	bound inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we present seven co-crystal structures of PDE4 and bound inhibitors that show the regulatory domain closed across the active site , thereby revealing the structural basis of PDE4 regulation .
	manualset3
86304	3	398422	5	NULL	NULL	0	NULL	regulatory domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we present seven co-crystal structures of PDE4 and bound inhibitors that show the regulatory domain closed across the active site , thereby revealing the structural basis of PDE4 regulation .
	manualset3
86305	4	398422	5	NULL	NULL	0	NULL	active site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we present seven co-crystal structures of PDE4 and bound inhibitors that show the regulatory domain closed across the active site , thereby revealing the structural basis of PDE4 regulation .
	manualset3
86306	5	398422	5	NULL	NULL	0	NULL	PDE4 regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we present seven co-crystal structures of PDE4 and bound inhibitors that show the regulatory domain closed across the active site , thereby revealing the structural basis of PDE4 regulation .
	manualset3
86307	1	398423	5	NULL	NULL	0	NULL	rationale	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we present the rationale and details of this approach , typical experimental results and necessary precautions .
	manualset3
86308	2	398423	5	NULL	NULL	0	NULL	typical experimental results	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we present the rationale and details of this approach , typical experimental results and necessary precautions .
	manualset3
86309	3	398423	5	NULL	NULL	0	NULL	necessary precautions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we present the rationale and details of this approach , typical experimental results and necessary precautions .
	manualset3
86310	1	398424	5	NULL	NULL	0	NULL	Val	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we propose that Val , Thr , and Ile are `` isosteric residues ' because they all contain a beta-branched side-chain .
	manualset3
86311	2	398424	5	NULL	NULL	0	NULL	Thr	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we propose that Val , Thr , and Ile are `` isosteric residues ' because they all contain a beta-branched side-chain .
	manualset3
86312	3	398424	5	NULL	NULL	0	NULL	Ile	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we propose that Val , Thr , and Ile are `` isosteric residues ' because they all contain a beta-branched side-chain .
	manualset3
86313	4	398424	5	NULL	NULL	0	NULL	isosteric residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we propose that Val , Thr , and Ile are `` isosteric residues ' because they all contain a beta-branched side-chain .
	manualset3
86314	5	398424	5	NULL	NULL	0	NULL	beta-branched side-chain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we propose that Val , Thr , and Ile are `` isosteric residues ' because they all contain a beta-branched side-chain .
	manualset3
86315	1	398425	5	NULL	NULL	NULL	NULL	sparse overcomplete linear representations	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we provide an example of how sparse overcomplete linear representations can directly solve difficult acoustic signal processing problems , using as an example monaural source separation using solely the cues provided by the differential filtering imposed on a source by its path from its origin to the cochlea ( the head-related transfer function ( HRTF ) ) .
	manualset3
86316	2	398425	5	NULL	NULL	NULL	NULL	acoustic signal processing	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we provide an example of how sparse overcomplete linear representations can directly solve difficult acoustic signal processing problems , using as an example monaural source separation using solely the cues provided by the differential filtering imposed on a source by its path from its origin to the cochlea ( the head-related transfer function ( HRTF ) ) .
	manualset3
86317	3	398425	5	NULL	NULL	0	NULL	monaural source separation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we provide an example of how sparse overcomplete linear representations can directly solve difficult acoustic signal processing problems , using as an example monaural source separation using solely the cues provided by the differential filtering imposed on a source by its path from its origin to the cochlea ( the head-related transfer function ( HRTF ) ) .
	manualset3
86318	4	398425	5	NULL	NULL	0	NULL	differential filtering	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we provide an example of how sparse overcomplete linear representations can directly solve difficult acoustic signal processing problems , using as an example monaural source separation using solely the cues provided by the differential filtering imposed on a source by its path from its origin to the cochlea ( the head-related transfer function ( HRTF ) ) .
	manualset3
86319	5	398425	5	NULL	NULL	0	NULL	cochlea	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we provide an example of how sparse overcomplete linear representations can directly solve difficult acoustic signal processing problems , using as an example monaural source separation using solely the cues provided by the differential filtering imposed on a source by its path from its origin to the cochlea ( the head-related transfer function ( HRTF ) ) .
	manualset3
86320	6	398425	5	NULL	NULL	0	NULL	head-related transfer function ( HRTF )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we provide an example of how sparse overcomplete linear representations can directly solve difficult acoustic signal processing problems , using as an example monaural source separation using solely the cues provided by the differential filtering imposed on a source by its path from its origin to the cochlea ( the head-related transfer function ( HRTF ) ) .
	manualset3
86321	1	398426	5	NULL	NULL	0	NULL	concentration-dependent interactions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we provide evidence that concentration-dependent interactions involving a network of these proteins are sufficient to determine the outcome of PKM splicing .
	manualset3
86322	2	398426	5	NULL	NULL	0	NULL	network	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we provide evidence that concentration-dependent interactions involving a network of these proteins are sufficient to determine the outcome of PKM splicing .
	manualset3
86323	3	398426	5	NULL	NULL	0	NULL	proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we provide evidence that concentration-dependent interactions involving a network of these proteins are sufficient to determine the outcome of PKM splicing .
	manualset3
86324	4	398426	5	NULL	NULL	0	NULL	PKM splicing	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we provide evidence that concentration-dependent interactions involving a network of these proteins are sufficient to determine the outcome of PKM splicing .
	manualset3
86325	1	398427	5	NULL	NULL	0	NULL	TFW-induced switch	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we provide evidence that the TFW-induced switch in Numb isoforms regulates Notch signaling strength and Notch target gene expression .
	manualset3
86326	2	398427	5	NULL	NULL	0	NULL	Numb isoforms	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we provide evidence that the TFW-induced switch in Numb isoforms regulates Notch signaling strength and Notch target gene expression .
	manualset3
86327	3	398427	5	NULL	NULL	0	NULL	Notch signaling strength	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we provide evidence that the TFW-induced switch in Numb isoforms regulates Notch signaling strength and Notch target gene expression .
	manualset3
86328	4	398427	5	NULL	NULL	0	NULL	Notch target gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we provide evidence that the TFW-induced switch in Numb isoforms regulates Notch signaling strength and Notch target gene expression .
	manualset3
86329	1	398428	5	NULL	NULL	0	NULL	Helix-Loop-Helix-COE transcription factor Collier	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we provide first molecular evidence that the Helix-Loop-Helix-COE transcription factor Collier fulfills this role by directly activating the expression of the segment polarity gene hedgehog in the posterior part of the intercalary segment .
	manualset3
86330	2	398428	5	NULL	NULL	0	NULL	expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we provide first molecular evidence that the Helix-Loop-Helix-COE transcription factor Collier fulfills this role by directly activating the expression of the segment polarity gene hedgehog in the posterior part of the intercalary segment .
	manualset3
86331	3	398428	5	NULL	NULL	0	NULL	segment polarity gene hedgehog	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we provide first molecular evidence that the Helix-Loop-Helix-COE transcription factor Collier fulfills this role by directly activating the expression of the segment polarity gene hedgehog in the posterior part of the intercalary segment .
	manualset3
86332	4	398428	5	NULL	NULL	0	NULL	posterior part of the intercalary segment	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we provide first molecular evidence that the Helix-Loop-Helix-COE transcription factor Collier fulfills this role by directly activating the expression of the segment polarity gene hedgehog in the posterior part of the intercalary segment .
	manualset3
86333	1	398429	5	NULL	NULL	0	NULL	4-year old female	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report a 4-year old female with idiopathic renal hypouricemia who presented with macroscopic hematuria due to obstructive calcium oxalate urolithiasis .
	manualset3
86334	2	398429	5	NULL	NULL	0	NULL	idiopathic renal hypouricemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report a 4-year old female with idiopathic renal hypouricemia who presented with macroscopic hematuria due to obstructive calcium oxalate urolithiasis .
	manualset3
86335	3	398429	5	NULL	NULL	0	NULL	macroscopic hematuria	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report a 4-year old female with idiopathic renal hypouricemia who presented with macroscopic hematuria due to obstructive calcium oxalate urolithiasis .
	manualset3
86336	4	398429	5	NULL	NULL	0	NULL	obstructive calcium oxalate urolithiasis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report a 4-year old female with idiopathic renal hypouricemia who presented with macroscopic hematuria due to obstructive calcium oxalate urolithiasis .
	manualset3
86337	1	398430	5	NULL	NULL	0	NULL	Susceptibilities of Pseudomonas species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Susceptibilities of Pseudomonas species to aminoglycosides and tetracyclines ) .
	manualset3
86338	2	398430	5	NULL	NULL	0	NULL	aminoglycosides	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Susceptibilities of Pseudomonas species to aminoglycosides and tetracyclines ) .
	manualset3
86339	3	398430	5	NULL	NULL	0	NULL	tetracyclines	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Susceptibilities of Pseudomonas species to aminoglycosides and tetracyclines ) .
	manualset3
85472	1	398431	14	13	NULL	NULL	NULL	novel conceptualisation	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we report a novel conceptualisation of impulsivity based on ` waiting ' and ` stopping ' efficiency with explanatory value in defining the psychological and neural basis of impulsivity and the high co-morbidity of brain disorders such as ADHD and drug addiction .
	manualset3
85474	3	398431	14	13	NULL	NULL	NULL	` waiting ' and ` stopping ' efficiency	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we report a novel conceptualisation of impulsivity based on ` waiting ' and ` stopping ' efficiency with explanatory value in defining the psychological and neural basis of impulsivity and the high co-morbidity of brain disorders such as ADHD and drug addiction .
	manualset3
85475	4	398431	14	13	NULL	NULL	NULL	psychological and neural basis of impulsivity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we report a novel conceptualisation of impulsivity based on ` waiting ' and ` stopping ' efficiency with explanatory value in defining the psychological and neural basis of impulsivity and the high co-morbidity of brain disorders such as ADHD and drug addiction .
	manualset3
85476	5	398431	14	13	NULL	0	NULL	 high co-morbidity of brain disorders 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report a novel conceptualisation of impulsivity based on ` waiting ' and ` stopping ' efficiency with explanatory value in defining the psychological and neural basis of impulsivity and the high co-morbidity of brain disorders such as ADHD and drug addiction .
	manualset3
85477	6	398431	14	13	NULL	NULL	NULL	ADHD	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we report a novel conceptualisation of impulsivity based on ` waiting ' and ` stopping ' efficiency with explanatory value in defining the psychological and neural basis of impulsivity and the high co-morbidity of brain disorders such as ADHD and drug addiction .
	manualset3
85478	7	398431	14	13	NULL	0	NULL	drug addiction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report a novel conceptualisation of impulsivity based on ` waiting ' and ` stopping ' efficiency with explanatory value in defining the psychological and neural basis of impulsivity and the high co-morbidity of brain disorders such as ADHD and drug addiction .
	manualset3
85500	2	398431	14	13	NULL	0	NULL	impulsivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report a novel conceptualisation of impulsivity based on ` waiting ' and ` stopping ' efficiency with explanatory value in defining the psychological and neural basis of impulsivity and the high co-morbidity of brain disorders such as ADHD and drug addiction .
	manualset3
85501	1	398432	14	13	NULL	0	NULL	general strategy	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report an unexpected and general strategy that is based on the requirement for specific cohorts of inhibitory histone methyltransferases ( HMTs ) to impose gene-specific gatekeeper functions that prevent unliganded nuclear receptors and other classes of regulated transcription factors from binding to their target gene promoters and causing constitutive gene activation in the absence of stimulating signals .
	manualset3
85502	2	398432	14	13	NULL	0	NULL	cohorts of inhibitory histone methyltransferases ( HMTs )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report an unexpected and general strategy that is based on the requirement for specific cohorts of inhibitory histone methyltransferases ( HMTs ) to impose gene-specific gatekeeper functions that prevent unliganded nuclear receptors and other classes of regulated transcription factors from binding to their target gene promoters and causing constitutive gene activation in the absence of stimulating signals .
	manualset3
85503	3	398432	14	13	NULL	0	NULL	gene-specific gatekeeper functions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report an unexpected and general strategy that is based on the requirement for specific cohorts of inhibitory histone methyltransferases ( HMTs ) to impose gene-specific gatekeeper functions that prevent unliganded nuclear receptors and other classes of regulated transcription factors from binding to their target gene promoters and causing constitutive gene activation in the absence of stimulating signals .
	manualset3
85504	4	398432	14	13	NULL	0	NULL	unliganded nuclear receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report an unexpected and general strategy that is based on the requirement for specific cohorts of inhibitory histone methyltransferases ( HMTs ) to impose gene-specific gatekeeper functions that prevent unliganded nuclear receptors and other classes of regulated transcription factors from binding to their target gene promoters and causing constitutive gene activation in the absence of stimulating signals .
	manualset3
85505	5	398432	14	13	NULL	0	NULL	classes of regulated transcription factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report an unexpected and general strategy that is based on the requirement for specific cohorts of inhibitory histone methyltransferases ( HMTs ) to impose gene-specific gatekeeper functions that prevent unliganded nuclear receptors and other classes of regulated transcription factors from binding to their target gene promoters and causing constitutive gene activation in the absence of stimulating signals .
	manualset3
85506	6	398432	14	13	NULL	0	NULL	 target gene promoters 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report an unexpected and general strategy that is based on the requirement for specific cohorts of inhibitory histone methyltransferases ( HMTs ) to impose gene-specific gatekeeper functions that prevent unliganded nuclear receptors and other classes of regulated transcription factors from binding to their target gene promoters and causing constitutive gene activation in the absence of stimulating signals .
	manualset3
85507	7	398432	14	13	NULL	NULL	NULL	 constitutive gene activation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we report an unexpected and general strategy that is based on the requirement for specific cohorts of inhibitory histone methyltransferases ( HMTs ) to impose gene-specific gatekeeper functions that prevent unliganded nuclear receptors and other classes of regulated transcription factors from binding to their target gene promoters and causing constitutive gene activation in the absence of stimulating signals .
	manualset3
85508	8	398432	14	13	NULL	0	NULL	stimulating signals	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report an unexpected and general strategy that is based on the requirement for specific cohorts of inhibitory histone methyltransferases ( HMTs ) to impose gene-specific gatekeeper functions that prevent unliganded nuclear receptors and other classes of regulated transcription factors from binding to their target gene promoters and causing constitutive gene activation in the absence of stimulating signals .
	manualset3
85511	1	398433	14	13	NULL	0	NULL	hypoxia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report effects of hypoxia on human monocyte-derived macrophage ( HMDM ) secreted glycosaminoglycans ( GAG ) , and its interaction with LDL .
	manualset3
85514	2	398433	14	13	NULL	0	NULL	human monocyte-derived macrophage ( HMDM )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report effects of hypoxia on human monocyte-derived macrophage ( HMDM ) secreted glycosaminoglycans ( GAG ) , and its interaction with LDL .
	manualset3
85525	3	398433	14	13	NULL	0	NULL	glycosaminoglycans ( GAG )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report effects of hypoxia on human monocyte-derived macrophage ( HMDM ) secreted glycosaminoglycans ( GAG ) , and its interaction with LDL .
	manualset3
85526	4	398433	14	13	NULL	0	NULL	interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report effects of hypoxia on human monocyte-derived macrophage ( HMDM ) secreted glycosaminoglycans ( GAG ) , and its interaction with LDL .
	manualset3
85527	5	398433	14	13	NULL	0	NULL	LDL 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report effects of hypoxia on human monocyte-derived macrophage ( HMDM ) secreted glycosaminoglycans ( GAG ) , and its interaction with LDL .
	manualset3
85528	1	398435	14	13	NULL	0	NULL	HOF1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report on the roles of HOF1 , BNI1 , and BNR1 in cytokinesis , focusing on Hof1p .
	manualset3
85529	2	398435	14	13	NULL	0	NULL	BNI1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report on the roles of HOF1 , BNI1 , and BNR1 in cytokinesis , focusing on Hof1p .
	manualset3
85530	3	398435	14	13	NULL	0	NULL	BNR1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report on the roles of HOF1 , BNI1 , and BNR1 in cytokinesis , focusing on Hof1p .
	manualset3
85531	4	398435	14	13	NULL	0	NULL	cytokinesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report on the roles of HOF1 , BNI1 , and BNR1 in cytokinesis , focusing on Hof1p .
	manualset3
85532	5	398435	14	13	NULL	0	NULL	Hof1p 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report on the roles of HOF1 , BNI1 , and BNR1 in cytokinesis , focusing on Hof1p .
	manualset3
85538	1	398436	14	13	NULL	0	NULL	mice infected with a recombinant spleen focus-forming retrovirus ( SFFV )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report that , in mice infected with a recombinant spleen focus-forming retrovirus ( SFFV ) expressing an oncogenic erythropoietin receptor ( EpoR ) , there was an increase in platelet count preceding the ensuing erythrocytosis .
	manualset3
85539	2	398436	14	13	NULL	0	NULL	oncogenic erythropoietin receptor ( EpoR )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report that , in mice infected with a recombinant spleen focus-forming retrovirus ( SFFV ) expressing an oncogenic erythropoietin receptor ( EpoR ) , there was an increase in platelet count preceding the ensuing erythrocytosis .
	manualset3
85540	3	398436	14	13	NULL	0	NULL	increase in platelet count	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report that , in mice infected with a recombinant spleen focus-forming retrovirus ( SFFV ) expressing an oncogenic erythropoietin receptor ( EpoR ) , there was an increase in platelet count preceding the ensuing erythrocytosis .
	manualset3
85541	4	398436	14	13	NULL	0	NULL	erythrocytosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report that , in mice infected with a recombinant spleen focus-forming retrovirus ( SFFV ) expressing an oncogenic erythropoietin receptor ( EpoR ) , there was an increase in platelet count preceding the ensuing erythrocytosis .
	manualset3
85542	1	398437	14	13	NULL	0	NULL	E2F-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report that E2F-1 is actively degraded by the ubiquitin-proteasome pathway .
	manualset3
85543	2	398437	14	13	NULL	0	NULL	ubiquitin-proteasome pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report that E2F-1 is actively degraded by the ubiquitin-proteasome pathway .
	manualset3
85544	1	398438	14	13	NULL	0	NULL	GATA-1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report that GATA-1 , SCL , and Klf1 form an erythroid core transcriptional network by co-occupying & gt ; 300 genes .
	manualset3
85545	2	398438	14	13	NULL	0	NULL	SCL	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report that GATA-1 , SCL , and Klf1 form an erythroid core transcriptional network by co-occupying & gt ; 300 genes .
	manualset3
85546	3	398438	14	13	NULL	0	NULL	Klf1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report that GATA-1 , SCL , and Klf1 form an erythroid core transcriptional network by co-occupying & gt ; 300 genes .
	manualset3
85547	4	398438	14	13	NULL	0	NULL	erythroid core transcriptional network	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report that GATA-1 , SCL , and Klf1 form an erythroid core transcriptional network by co-occupying & gt ; 300 genes .
	manualset3
85548	5	398438	14	13	NULL	NULL	NULL	300 genes	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we report that GATA-1 , SCL , and Klf1 form an erythroid core transcriptional network by co-occupying & gt ; 300 genes .
	manualset3
85549	1	398439	14	13	NULL	0	NULL	HSV type 1 ( HSV-1 )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report that HSV type 1 ( HSV-1 ) induces persistent activation of transcription factor NF-kappa B , a critical regulator of genes involved in inflammation , by activating the I kappa B kinase ( IKK ) in the early phase of infection .
	manualset3
85550	2	398439	14	13	NULL	NULL	NULL	activation of transcription factor 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we report that HSV type 1 ( HSV-1 ) induces persistent activation of transcription factor NF-kappa B , a critical regulator of genes involved in inflammation , by activating the I kappa B kinase ( IKK ) in the early phase of infection .
	manualset3
85551	4	398439	14	13	NULL	NULL	NULL	critical regulator of genes 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we report that HSV type 1 ( HSV-1 ) induces persistent activation of transcription factor NF-kappa B , a critical regulator of genes involved in inflammation , by activating the I kappa B kinase ( IKK ) in the early phase of infection .
	manualset3
85552	5	398439	14	13	NULL	NULL	NULL	 inflammation 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we report that HSV type 1 ( HSV-1 ) induces persistent activation of transcription factor NF-kappa B , a critical regulator of genes involved in inflammation , by activating the I kappa B kinase ( IKK ) in the early phase of infection .
	manualset3
85553	6	398439	14	13	NULL	NULL	NULL	activating the I kappa B kinase ( IKK )	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we report that HSV type 1 ( HSV-1 ) induces persistent activation of transcription factor NF-kappa B , a critical regulator of genes involved in inflammation , by activating the I kappa B kinase ( IKK ) in the early phase of infection .
	manualset3
85554	7	398439	14	13	NULL	NULL	NULL	early phase	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we report that HSV type 1 ( HSV-1 ) induces persistent activation of transcription factor NF-kappa B , a critical regulator of genes involved in inflammation , by activating the I kappa B kinase ( IKK ) in the early phase of infection .
	manualset3
85555	8	398439	14	13	NULL	NULL	NULL	infection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we report that HSV type 1 ( HSV-1 ) induces persistent activation of transcription factor NF-kappa B , a critical regulator of genes involved in inflammation , by activating the I kappa B kinase ( IKK ) in the early phase of infection .
	manualset3
86124	3	398439	14	13	NULL	0	NULL	NF-kappa B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report that HSV type 1 ( HSV-1 ) induces persistent activation of transcription factor NF-kappa B , a critical regulator of genes involved in inflammation , by activating the I kappa B kinase ( IKK ) in the early phase of infection .
	manualset3
85556	1	398440	14	13	NULL	NULL	NULL	endogenous local signaling	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we report that only endogenous local signaling at D ( 1 ) dopamine receptors is needed for rostral generation of excessive eating , potentially implicating a direct output pathway contribution .
	manualset3
85557	2	398440	14	13	NULL	0	NULL	 D ( 1 ) dopamine receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report that only endogenous local signaling at D ( 1 ) dopamine receptors is needed for rostral generation of excessive eating , potentially implicating a direct output pathway contribution .
	manualset3
85558	3	398440	14	13	NULL	NULL	NULL	rostral generation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we report that only endogenous local signaling at D ( 1 ) dopamine receptors is needed for rostral generation of excessive eating , potentially implicating a direct output pathway contribution .
	manualset3
85559	5	398440	14	13	NULL	NULL	NULL	output pathway	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we report that only endogenous local signaling at D ( 1 ) dopamine receptors is needed for rostral generation of excessive eating , potentially implicating a direct output pathway contribution .
	manualset3
86125	4	398440	14	13	NULL	0	NULL	excessive eating	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report that only endogenous local signaling at D ( 1 ) dopamine receptors is needed for rostral generation of excessive eating , potentially implicating a direct output pathway contribution .
	manualset3
85560	1	398441	14	13	NULL	0	NULL	crystal structure	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report the crystal structure of a squid core complexin-SNARE complex at 2.95-A resolution .
	manualset3
85561	2	398441	14	13	NULL	0	NULL	squid core complexin-SNARE complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report the crystal structure of a squid core complexin-SNARE complex at 2.95-A resolution .
	manualset3
85562	3	398441	14	13	NULL	0	NULL	2.95-A resolution	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report the crystal structure of a squid core complexin-SNARE complex at 2.95-A resolution .
	manualset3
85563	1	398442	14	13	NULL	0	NULL	crystal structure	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report the crystal structure of the kinase domain of SnRK2 .6 at 2.6 - resolution .
	manualset3
85564	2	398442	14	13	NULL	0	NULL	kinase domain of SnRK2 .6	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report the crystal structure of the kinase domain of SnRK2 .6 at 2.6 - resolution .
	manualset3
85565	3	398442	14	13	NULL	0	NULL	2.6 - resolution 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report the crystal structure of the kinase domain of SnRK2 .6 at 2.6 - resolution .
	manualset3
85566	1	398443	14	13	NULL	0	NULL	optimisation of immunofluorescent staining	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report the optimisation of immunofluorescent staining for cell surface and intracellular antigens using three-colour flow cytometric analysis to measure the frequency of rat CD3 ( + ) 4 ( + ) T-cells that produce IFN-gamma , IL-4 and IL-10 .
	manualset3
85567	2	398443	14	13	NULL	NULL	NULL	cell surface antigens	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we report the optimisation of immunofluorescent staining for cell surface and intracellular antigens using three-colour flow cytometric analysis to measure the frequency of rat CD3 ( + ) 4 ( + ) T-cells that produce IFN-gamma , IL-4 and IL-10 .
	manualset3
85568	3	398443	14	13	NULL	0	NULL	three-colour flow cytometric analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report the optimisation of immunofluorescent staining for cell surface and intracellular antigens using three-colour flow cytometric analysis to measure the frequency of rat CD3 ( + ) 4 ( + ) T-cells that produce IFN-gamma , IL-4 and IL-10 .
	manualset3
85569	4	398443	14	13	NULL	0	NULL	rat CD3 ( + ) 4 ( + ) T-cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report the optimisation of immunofluorescent staining for cell surface and intracellular antigens using three-colour flow cytometric analysis to measure the frequency of rat CD3 ( + ) 4 ( + ) T-cells that produce IFN-gamma , IL-4 and IL-10 .
	manualset3
85570	5	398443	14	13	NULL	0	NULL	IFN-gamma	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report the optimisation of immunofluorescent staining for cell surface and intracellular antigens using three-colour flow cytometric analysis to measure the frequency of rat CD3 ( + ) 4 ( + ) T-cells that produce IFN-gamma , IL-4 and IL-10 .
	manualset3
85571	6	398443	14	13	NULL	0	NULL	IL-4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report the optimisation of immunofluorescent staining for cell surface and intracellular antigens using three-colour flow cytometric analysis to measure the frequency of rat CD3 ( + ) 4 ( + ) T-cells that produce IFN-gamma , IL-4 and IL-10 .
	manualset3
85572	7	398443	14	13	NULL	0	NULL	 IL-10	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report the optimisation of immunofluorescent staining for cell surface and intracellular antigens using three-colour flow cytometric analysis to measure the frequency of rat CD3 ( + ) 4 ( + ) T-cells that produce IFN-gamma , IL-4 and IL-10 .
	manualset3
86126	8	398443	14	13	NULL	0	NULL	intracellular antigens	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report the optimisation of immunofluorescent staining for cell surface and intracellular antigens using three-colour flow cytometric analysis to measure the frequency of rat CD3 ( + ) 4 ( + ) T-cells that produce IFN-gamma , IL-4 and IL-10 .
	manualset3
85573	1	398444	14	13	NULL	0	NULL	resection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report the successful complete resection of a giant , local recurrent chondrosarcoma of the chest wall ( max .
	manualset3
85574	2	398444	14	13	NULL	0	NULL	 giant , local recurrent chondrosarcoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report the successful complete resection of a giant , local recurrent chondrosarcoma of the chest wall ( max .
	manualset3
85575	3	398444	14	13	NULL	0	NULL	chest wall 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report the successful complete resection of a giant , local recurrent chondrosarcoma of the chest wall ( max .
	manualset3
85634	1	398445	14	13	NULL	0	NULL	three types	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report three types of responses to EFS in human isolated colon circular muscle : monophasic cholinergic contraction during EFS , biphasic response ( nitrergic relaxation during EFS followed by cholinergic contraction after termination of EFS ) and triphasic response ( cholinergic contraction followed by nitrergic relaxation during EFS and a tachykininergic contraction after EFS ) .
	manualset3
85636	3	398445	14	13	NULL	NULL	NULL	human isolated colon circular muscle	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we report three types of responses to EFS in human isolated colon circular muscle : monophasic cholinergic contraction during EFS , biphasic response ( nitrergic relaxation during EFS followed by cholinergic contraction after termination of EFS ) and triphasic response ( cholinergic contraction followed by nitrergic relaxation during EFS and a tachykininergic contraction after EFS ) .
	manualset3
85637	4	398445	14	13	NULL	NULL	NULL	monophasic cholinergic contraction during EFS 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we report three types of responses to EFS in human isolated colon circular muscle : monophasic cholinergic contraction during EFS , biphasic response ( nitrergic relaxation during EFS followed by cholinergic contraction after termination of EFS ) and triphasic response ( cholinergic contraction followed by nitrergic relaxation during EFS and a tachykininergic contraction after EFS ) .
	manualset3
85639	6	398445	14	13	NULL	0	NULL	biphasic response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report three types of responses to EFS in human isolated colon circular muscle : monophasic cholinergic contraction during EFS , biphasic response ( nitrergic relaxation during EFS followed by cholinergic contraction after termination of EFS ) and triphasic response ( cholinergic contraction followed by nitrergic relaxation during EFS and a tachykininergic contraction after EFS ) .
	manualset3
85640	7	398445	14	13	NULL	NULL	NULL	nitrergic relaxation during EFS	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we report three types of responses to EFS in human isolated colon circular muscle : monophasic cholinergic contraction during EFS , biphasic response ( nitrergic relaxation during EFS followed by cholinergic contraction after termination of EFS ) and triphasic response ( cholinergic contraction followed by nitrergic relaxation during EFS and a tachykininergic contraction after EFS ) .
	manualset3
85641	8	398445	14	13	NULL	0	NULL	cholinergic contraction after termination of EFS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report three types of responses to EFS in human isolated colon circular muscle : monophasic cholinergic contraction during EFS , biphasic response ( nitrergic relaxation during EFS followed by cholinergic contraction after termination of EFS ) and triphasic response ( cholinergic contraction followed by nitrergic relaxation during EFS and a tachykininergic contraction after EFS ) .
	manualset3
85642	9	398445	14	13	NULL	0	NULL	triphasic response 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report three types of responses to EFS in human isolated colon circular muscle : monophasic cholinergic contraction during EFS , biphasic response ( nitrergic relaxation during EFS followed by cholinergic contraction after termination of EFS ) and triphasic response ( cholinergic contraction followed by nitrergic relaxation during EFS and a tachykininergic contraction after EFS ) .
	manualset3
85643	10	398445	14	13	NULL	0	NULL	cholinergic contraction followed by nitrergic relaxation during EFS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report three types of responses to EFS in human isolated colon circular muscle : monophasic cholinergic contraction during EFS , biphasic response ( nitrergic relaxation during EFS followed by cholinergic contraction after termination of EFS ) and triphasic response ( cholinergic contraction followed by nitrergic relaxation during EFS and a tachykininergic contraction after EFS ) .
	manualset3
85644	11	398445	14	13	NULL	0	NULL	tachykininergic contraction after EFS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report three types of responses to EFS in human isolated colon circular muscle : monophasic cholinergic contraction during EFS , biphasic response ( nitrergic relaxation during EFS followed by cholinergic contraction after termination of EFS ) and triphasic response ( cholinergic contraction followed by nitrergic relaxation during EFS and a tachykininergic contraction after EFS ) .
	manualset3
86127	2	398445	14	13	NULL	NULL	NULL	responses to EFS	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we report three types of responses to EFS in human isolated colon circular muscle : monophasic cholinergic contraction during EFS , biphasic response ( nitrergic relaxation during EFS followed by cholinergic contraction after termination of EFS ) and triphasic response ( cholinergic contraction followed by nitrergic relaxation during EFS and a tachykininergic contraction after EFS ) .
	manualset3
85653	1	398448	14	13	NULL	NULL	NULL	non-native fish pathogens	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we review the most important non-native fish and shellfish pathogens in European waters and their global impacts on wild fish host populations .
	manualset3
85654	2	398448	14	13	NULL	0	NULL	shellfish pathogens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we review the most important non-native fish and shellfish pathogens in European waters and their global impacts on wild fish host populations .
	manualset3
85655	3	398448	14	13	NULL	0	NULL	European waters	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we review the most important non-native fish and shellfish pathogens in European waters and their global impacts on wild fish host populations .
	manualset3
85656	4	398448	14	13	NULL	0	NULL	wild fish host populations 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we review the most important non-native fish and shellfish pathogens in European waters and their global impacts on wild fish host populations .
	manualset3
85657	1	398449	14	13	NULL	0	NULL	Stat-1 nuclear accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show inhibition of Stat-1 nuclear accumulation in cells that express ICP27 .
	manualset3
85658	2	398449	14	13	NULL	0	NULL	 cells that express ICP27	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show inhibition of Stat-1 nuclear accumulation in cells that express ICP27 .
	manualset3
85659	1	398450	14	13	NULL	NULL	NULL	Synergistic protective effect of testicular cells	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Synergistic protective effect of testicular cells expressing Fas ligand and cyclosporine A on the survival of islet allografts ) .
	manualset3
85663	2	398450	14	13	NULL	0	NULL	 Fas ligand	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Synergistic protective effect of testicular cells expressing Fas ligand and cyclosporine A on the survival of islet allografts ) .
	manualset3
85665	3	398450	14	13	NULL	0	NULL	cyclosporine A	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Synergistic protective effect of testicular cells expressing Fas ligand and cyclosporine A on the survival of islet allografts ) .
	manualset3
85667	4	398450	14	13	NULL	0	NULL	survival of islet allografts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Synergistic protective effect of testicular cells expressing Fas ligand and cyclosporine A on the survival of islet allografts ) .
	manualset3
85668	1	398451	14	13	NULL	0	NULL	 ADC protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that ADC protein was increasingly expressed at early stages of hop internode culture ( 12h ) .
	manualset3
85669	2	398451	14	13	NULL	0	NULL	early stages	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that ADC protein was increasingly expressed at early stages of hop internode culture ( 12h ) .
	manualset3
85671	3	398451	14	13	NULL	0	NULL	hop internode culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that ADC protein was increasingly expressed at early stages of hop internode culture ( 12h ) .
	manualset3
85672	4	398451	14	13	NULL	0	NULL	12h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that ADC protein was increasingly expressed at early stages of hop internode culture ( 12h ) .
	manualset3
85673	1	398452	14	13	NULL	0	NULL	AcrS	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that AcrS represses other multidrug efflux genes , acrAB , which encode a major efflux system in Escherichia coli .
	manualset3
85676	2	398452	14	13	NULL	0	NULL	multidrug efflux genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that AcrS represses other multidrug efflux genes , acrAB , which encode a major efflux system in Escherichia coli .
	manualset3
85678	3	398452	14	13	NULL	0	NULL	acrAB	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that AcrS represses other multidrug efflux genes , acrAB , which encode a major efflux system in Escherichia coli .
	manualset3
85680	4	398452	14	13	NULL	0	NULL	major efflux system	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that AcrS represses other multidrug efflux genes , acrAB , which encode a major efflux system in Escherichia coli .
	manualset3
85681	5	398452	14	13	NULL	0	NULL	Escherichia coli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that AcrS represses other multidrug efflux genes , acrAB , which encode a major efflux system in Escherichia coli .
	manualset3
85682	1	398453	14	13	NULL	0	NULL	Ad-specific CTLs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that Ad-specific CTLs recognize the early region 2 proteins DNA polymerase ( Pol ) and DNA-binding protein ( DBP ) .
	manualset3
85683	2	398453	14	13	NULL	NULL	NULL	2	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we show that Ad-specific CTLs recognize the early region 2 proteins DNA polymerase ( Pol ) and DNA-binding protein ( DBP ) .
	manualset3
85684	3	398453	14	13	NULL	0	NULL	 DNA polymerase ( Pol )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that Ad-specific CTLs recognize the early region 2 proteins DNA polymerase ( Pol ) and DNA-binding protein ( DBP ) .
	manualset3
85685	4	398453	14	13	NULL	0	NULL	DNA-binding protein ( DBP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that Ad-specific CTLs recognize the early region 2 proteins DNA polymerase ( Pol ) and DNA-binding protein ( DBP ) .
	manualset3
86130	2	398453	14	13	NULL	0	NULL	proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that Ad-specific CTLs recognize the early region 2 proteins DNA polymerase ( Pol ) and DNA-binding protein ( DBP ) .
	manualset3
85686	1	398454	14	13	NULL	0	NULL	CD94	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that CD94 , a molecule preferentially expressed by NK cells , is essential for the resistance of C57BL/6 mice to mousepox , a disease caused by the Orthopoxvirus ectromelia virus .
	manualset3
85687	2	398454	14	13	NULL	0	NULL	molecule preferentially expressed	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that CD94 , a molecule preferentially expressed by NK cells , is essential for the resistance of C57BL/6 mice to mousepox , a disease caused by the Orthopoxvirus ectromelia virus .
	manualset3
85688	3	398454	14	13	NULL	0	NULL	NK cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that CD94 , a molecule preferentially expressed by NK cells , is essential for the resistance of C57BL/6 mice to mousepox , a disease caused by the Orthopoxvirus ectromelia virus .
	manualset3
85689	4	398454	14	13	NULL	0	NULL	resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that CD94 , a molecule preferentially expressed by NK cells , is essential for the resistance of C57BL/6 mice to mousepox , a disease caused by the Orthopoxvirus ectromelia virus .
	manualset3
85690	5	398454	14	13	NULL	0	NULL	C57BL/6 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that CD94 , a molecule preferentially expressed by NK cells , is essential for the resistance of C57BL/6 mice to mousepox , a disease caused by the Orthopoxvirus ectromelia virus .
	manualset3
85691	6	398454	14	13	NULL	0	NULL	mousepox	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that CD94 , a molecule preferentially expressed by NK cells , is essential for the resistance of C57BL/6 mice to mousepox , a disease caused by the Orthopoxvirus ectromelia virus .
	manualset3
85692	7	398454	14	13	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that CD94 , a molecule preferentially expressed by NK cells , is essential for the resistance of C57BL/6 mice to mousepox , a disease caused by the Orthopoxvirus ectromelia virus .
	manualset3
85693	8	398454	14	13	NULL	0	NULL	Orthopoxvirus ectromelia virus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that CD94 , a molecule preferentially expressed by NK cells , is essential for the resistance of C57BL/6 mice to mousepox , a disease caused by the Orthopoxvirus ectromelia virus .
	manualset3
85694	1	398455	14	13	NULL	NULL	NULL	HA scaffolds	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we show that HA scaffolds were stable cell carriers and had the potential to generate volume-retaining tissue .
	manualset3
85696	2	398455	14	13	NULL	NULL	NULL	volume-retaining tissue	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we show that HA scaffolds were stable cell carriers and had the potential to generate volume-retaining tissue .
	manualset3
85700	1	398456	14	13	NULL	0	NULL	 LPS	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that LPS induces nuclear expression of c-Rel/p50 heterodimers as well as p50/p65 ( NF-kappa B ) kappa B DNA-binding complexes in human monocytic THP-1 cells .
	manualset3
85701	2	398456	14	13	NULL	0	NULL	nuclear expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that LPS induces nuclear expression of c-Rel/p50 heterodimers as well as p50/p65 ( NF-kappa B ) kappa B DNA-binding complexes in human monocytic THP-1 cells .
	manualset3
85702	3	398456	14	13	NULL	NULL	NULL	c-Rel/p50 heterodimers	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we show that LPS induces nuclear expression of c-Rel/p50 heterodimers as well as p50/p65 ( NF-kappa B ) kappa B DNA-binding complexes in human monocytic THP-1 cells .
	manualset3
85703	4	398456	14	13	NULL	0	NULL	p50/p65 ( NF-kappa B ) kappa B DNA-binding complexes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that LPS induces nuclear expression of c-Rel/p50 heterodimers as well as p50/p65 ( NF-kappa B ) kappa B DNA-binding complexes in human monocytic THP-1 cells .
	manualset3
85704	5	398456	14	13	NULL	0	NULL	human monocytic THP-1 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that LPS induces nuclear expression of c-Rel/p50 heterodimers as well as p50/p65 ( NF-kappa B ) kappa B DNA-binding complexes in human monocytic THP-1 cells .
	manualset3
85705	1	398457	14	13	NULL	NULL	NULL	MLS0315771	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we show that MLS0315771 , a potent MPI inhibitor from the benzoisothiazolone series , diverts Man-6-P toward glycosylation in various cell lines including fibroblasts from CDG-Ia patients and improves N-glycosylation .
	manualset3
85706	2	398457	14	13	NULL	NULL	NULL	MPI inhibitor	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we show that MLS0315771 , a potent MPI inhibitor from the benzoisothiazolone series , diverts Man-6-P toward glycosylation in various cell lines including fibroblasts from CDG-Ia patients and improves N-glycosylation .
	manualset3
85707	3	398457	14	13	NULL	NULL	NULL	 benzoisothiazolone series	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we show that MLS0315771 , a potent MPI inhibitor from the benzoisothiazolone series , diverts Man-6-P toward glycosylation in various cell lines including fibroblasts from CDG-Ia patients and improves N-glycosylation .
	manualset3
85708	4	398457	14	13	NULL	NULL	NULL	Man-6-P	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we show that MLS0315771 , a potent MPI inhibitor from the benzoisothiazolone series , diverts Man-6-P toward glycosylation in various cell lines including fibroblasts from CDG-Ia patients and improves N-glycosylation .
	manualset3
85709	5	398457	14	13	NULL	NULL	NULL	glycosylation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we show that MLS0315771 , a potent MPI inhibitor from the benzoisothiazolone series , diverts Man-6-P toward glycosylation in various cell lines including fibroblasts from CDG-Ia patients and improves N-glycosylation .
	manualset3
85710	6	398457	14	13	NULL	NULL	NULL	various cell lines 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we show that MLS0315771 , a potent MPI inhibitor from the benzoisothiazolone series , diverts Man-6-P toward glycosylation in various cell lines including fibroblasts from CDG-Ia patients and improves N-glycosylation .
	manualset3
85711	7	398457	14	13	NULL	0	NULL	fibroblasts 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that MLS0315771 , a potent MPI inhibitor from the benzoisothiazolone series , diverts Man-6-P toward glycosylation in various cell lines including fibroblasts from CDG-Ia patients and improves N-glycosylation .
	manualset3
85712	8	398457	14	13	NULL	0	NULL	CDG-Ia patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that MLS0315771 , a potent MPI inhibitor from the benzoisothiazolone series , diverts Man-6-P toward glycosylation in various cell lines including fibroblasts from CDG-Ia patients and improves N-glycosylation .
	manualset3
85713	9	398457	14	13	NULL	0	NULL	N-glycosylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that MLS0315771 , a potent MPI inhibitor from the benzoisothiazolone series , diverts Man-6-P toward glycosylation in various cell lines including fibroblasts from CDG-Ia patients and improves N-glycosylation .
	manualset3
85714	1	398458	14	13	NULL	0	NULL	mutations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that both mutations constitutively activate the mammalian target of rapamycin ( mTOR ) signaling pathway .
	manualset3
85715	2	398458	14	13	NULL	0	NULL	mammalian target of rapamycin ( mTOR ) signaling pathway 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that both mutations constitutively activate the mammalian target of rapamycin ( mTOR ) signaling pathway .
	manualset3
85716	1	398459	14	13	NULL	0	NULL	chimeric PRL receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that chimeric PRL receptors that contain the transmembrane and cytoplasmic domains of the IL-2R beta or beta c-chains transduce in response to PRL tyrosine phosphorylation and activation of Jak1 and Jak2 , respectively .
	manualset3
85717	2	398459	14	13	NULL	0	NULL	transmembrane domains of the IL-2R beta or beta c-chains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that chimeric PRL receptors that contain the transmembrane and cytoplasmic domains of the IL-2R beta or beta c-chains transduce in response to PRL tyrosine phosphorylation and activation of Jak1 and Jak2 , respectively .
	manualset3
85718	3	398459	14	13	NULL	0	NULL	cytoplasmic domains of the IL-2R beta or beta c-chains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that chimeric PRL receptors that contain the transmembrane and cytoplasmic domains of the IL-2R beta or beta c-chains transduce in response to PRL tyrosine phosphorylation and activation of Jak1 and Jak2 , respectively .
	manualset3
85719	4	398459	14	13	NULL	0	NULL	PRL tyrosine phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that chimeric PRL receptors that contain the transmembrane and cytoplasmic domains of the IL-2R beta or beta c-chains transduce in response to PRL tyrosine phosphorylation and activation of Jak1 and Jak2 , respectively .
	manualset3
85720	5	398459	14	13	NULL	0	NULL	activation of Jak1 and Jak2	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that chimeric PRL receptors that contain the transmembrane and cytoplasmic domains of the IL-2R beta or beta c-chains transduce in response to PRL tyrosine phosphorylation and activation of Jak1 and Jak2 , respectively .
	manualset3
85721	1	398460	14	13	NULL	0	NULL	clam p82 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that clam p82 is related to Xenopus CPEB , an RNA-binding protein that interacts with the U-rich cytoplasmic polyadenylation elements ( CPEs ) of maternal mRNAs and promotes their polyadenylation .
	manualset3
85722	2	398460	14	13	NULL	0	NULL	Xenopus CPEB	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that clam p82 is related to Xenopus CPEB , an RNA-binding protein that interacts with the U-rich cytoplasmic polyadenylation elements ( CPEs ) of maternal mRNAs and promotes their polyadenylation .
	manualset3
85723	3	398460	14	13	NULL	0	NULL	RNA-binding protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that clam p82 is related to Xenopus CPEB , an RNA-binding protein that interacts with the U-rich cytoplasmic polyadenylation elements ( CPEs ) of maternal mRNAs and promotes their polyadenylation .
	manualset3
85724	4	398460	14	13	NULL	0	NULL	U-rich cytoplasmic polyadenylation elements ( CPEs ) of maternal mRNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that clam p82 is related to Xenopus CPEB , an RNA-binding protein that interacts with the U-rich cytoplasmic polyadenylation elements ( CPEs ) of maternal mRNAs and promotes their polyadenylation .
	manualset3
85725	5	398460	14	13	NULL	0	NULL	polyadenylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that clam p82 is related to Xenopus CPEB , an RNA-binding protein that interacts with the U-rich cytoplasmic polyadenylation elements ( CPEs ) of maternal mRNAs and promotes their polyadenylation .
	manualset3
85726	1	398461	14	13	NULL	0	NULL	 commensal microbiota 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that encounter with commensal microbiota results in the peripheral generation of T ( reg ) cells rather than pathogenic effectors .
	manualset3
85727	2	398461	14	13	NULL	0	NULL	peripheral generation of T ( reg ) cells 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that encounter with commensal microbiota results in the peripheral generation of T ( reg ) cells rather than pathogenic effectors .
	manualset3
85728	3	398461	14	13	NULL	0	NULL	pathogenic effectors	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that encounter with commensal microbiota results in the peripheral generation of T ( reg ) cells rather than pathogenic effectors .
	manualset3
85729	1	398462	14	13	NULL	0	NULL	mTOR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that mTOR is necessary for the maintenance of mitochondrial oxidative function .
	manualset3
85730	2	398462	14	13	NULL	NULL	NULL	maintenance of mitochondrial oxidative function function 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we show that mTOR is necessary for the maintenance of mitochondrial oxidative function .
	manualset3
85731	1	398463	14	13	NULL	NULL	NULL	Mcm proteins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we show that the Mcm proteins of budding yeast are abundant and are quantitatively found in a chromatin-enriched fraction specifically during the G1 phase of the cell cycle .
	manualset3
85732	2	398463	14	13	NULL	0	NULL	budding yeast	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that the Mcm proteins of budding yeast are abundant and are quantitatively found in a chromatin-enriched fraction specifically during the G1 phase of the cell cycle .
	manualset3
85733	3	398463	14	13	NULL	0	NULL	chromatin-enriched fraction 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that the Mcm proteins of budding yeast are abundant and are quantitatively found in a chromatin-enriched fraction specifically during the G1 phase of the cell cycle .
	manualset3
85734	4	398463	14	13	NULL	0	NULL	G1 phase of the cell cycle	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that the Mcm proteins of budding yeast are abundant and are quantitatively found in a chromatin-enriched fraction specifically during the G1 phase of the cell cycle .
	manualset3
85735	1	398464	14	13	NULL	NULL	NULL	color octet mechanism 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we show that the color octet mechanism reproduces the RHIC data for J/psi production in pp collisions with respect to the p ( T ) distribution , the rapidity distribution , and the total cross section at square root = 200 GeV .
	manualset3
85736	2	398464	14	13	NULL	NULL	NULL	data 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we show that the color octet mechanism reproduces the RHIC data for J/psi production in pp collisions with respect to the p ( T ) distribution , the rapidity distribution , and the total cross section at square root = 200 GeV .
	manualset3
85737	6	398464	14	13	NULL	NULL	NULL	square root = 200 GeV	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we show that the color octet mechanism reproduces the RHIC data for J/psi production in pp collisions with respect to the p ( T ) distribution , the rapidity distribution , and the total cross section at square root = 200 GeV .
	manualset3
86131	3	398464	14	13	NULL	NULL	NULL	J/psi production 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we show that the color octet mechanism reproduces the RHIC data for J/psi production in pp collisions with respect to the p ( T ) distribution , the rapidity distribution , and the total cross section at square root = 200 GeV .
	manualset3
86132	4	398464	14	13	NULL	NULL	NULL	pp collisions	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we show that the color octet mechanism reproduces the RHIC data for J/psi production in pp collisions with respect to the p ( T ) distribution , the rapidity distribution , and the total cross section at square root = 200 GeV .
	manualset3
86133	5	398464	14	13	NULL	NULL	NULL	p ( T ) distribution	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we show that the color octet mechanism reproduces the RHIC data for J/psi production in pp collisions with respect to the p ( T ) distribution , the rapidity distribution , and the total cross section at square root = 200 GeV .
	manualset3
86143	7	398464	14	13	NULL	0	NULL	RHIC	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that the color octet mechanism reproduces the RHIC data for J/psi production in pp collisions with respect to the p ( T ) distribution , the rapidity distribution , and the total cross section at square root = 200 GeV .
	manualset3
86144	8	398464	14	13	NULL	0	NULL	rapidity distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that the color octet mechanism reproduces the RHIC data for J/psi production in pp collisions with respect to the p ( T ) distribution , the rapidity distribution , and the total cross section at square root = 200 GeV .
	manualset3
86145	9	398464	14	13	NULL	0	NULL	total cross section	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that the color octet mechanism reproduces the RHIC data for J/psi production in pp collisions with respect to the p ( T ) distribution , the rapidity distribution , and the total cross section at square root = 200 GeV .
	manualset3
85738	1	398465	14	13	NULL	0	NULL	neoplastic cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that the neoplastic cells of many human breast cancers express the ROR1 protein and high-level expression of ROR1 in breast adenocarcinoma was associated with aggressive disease .
	manualset3
85739	2	398465	14	13	NULL	0	NULL	human breast cancers	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that the neoplastic cells of many human breast cancers express the ROR1 protein and high-level expression of ROR1 in breast adenocarcinoma was associated with aggressive disease .
	manualset3
85740	3	398465	14	13	NULL	0	NULL	ROR1 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that the neoplastic cells of many human breast cancers express the ROR1 protein and high-level expression of ROR1 in breast adenocarcinoma was associated with aggressive disease .
	manualset3
85741	4	398465	14	13	NULL	0	NULL	high-level expression of ROR1	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that the neoplastic cells of many human breast cancers express the ROR1 protein and high-level expression of ROR1 in breast adenocarcinoma was associated with aggressive disease .
	manualset3
85742	5	398465	14	13	NULL	0	NULL	breast adenocarcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that the neoplastic cells of many human breast cancers express the ROR1 protein and high-level expression of ROR1 in breast adenocarcinoma was associated with aggressive disease .
	manualset3
85743	6	398465	14	13	NULL	0	NULL	aggressive disease	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that the neoplastic cells of many human breast cancers express the ROR1 protein and high-level expression of ROR1 in breast adenocarcinoma was associated with aggressive disease .
	manualset3
85744	1	398466	14	13	NULL	0	NULL	vitellogenin mRNA-binding protein ( VitRNABP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that the vitellogenin mRNA-binding protein ( VitRNABP ) is vigilin .
	manualset3
85745	2	398466	14	13	NULL	0	NULL	vigilin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we show that the vitellogenin mRNA-binding protein ( VitRNABP ) is vigilin .
	manualset3
85746	1	398467	14	13	NULL	0	NULL	human insulin ( HI )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we studied the role of human insulin ( HI ) in breast milk as a modulator of the immune response to insulin .
	manualset3
85747	2	398467	14	13	NULL	NULL	NULL	breast milk 	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we studied the role of human insulin ( HI ) in breast milk as a modulator of the immune response to insulin .
	manualset3
85748	3	398467	14	13	NULL	0	NULL	immune response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we studied the role of human insulin ( HI ) in breast milk as a modulator of the immune response to insulin .
	manualset3
85749	4	398467	14	13	NULL	0	NULL	 insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we studied the role of human insulin ( HI ) in breast milk as a modulator of the immune response to insulin .
	manualset3
85752	1	398468	14	13	NULL	0	NULL	pattern of expression of certain genes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we summarise the pattern of expression of certain genes involved in the eye network that have been isolated in planarians , such as Otx , Pax-6 , Six , Rax and opsin .
	manualset3
85753	2	398468	14	13	NULL	0	NULL	eye network	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we summarise the pattern of expression of certain genes involved in the eye network that have been isolated in planarians , such as Otx , Pax-6 , Six , Rax and opsin .
	manualset3
85754	3	398468	14	13	NULL	0	NULL	planarians	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we summarise the pattern of expression of certain genes involved in the eye network that have been isolated in planarians , such as Otx , Pax-6 , Six , Rax and opsin .
	manualset3
85755	4	398468	14	13	NULL	0	NULL	Otx	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we summarise the pattern of expression of certain genes involved in the eye network that have been isolated in planarians , such as Otx , Pax-6 , Six , Rax and opsin .
	manualset3
85756	5	398468	14	13	NULL	0	NULL	Pax-6	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we summarise the pattern of expression of certain genes involved in the eye network that have been isolated in planarians , such as Otx , Pax-6 , Six , Rax and opsin .
	manualset3
85757	6	398468	14	13	NULL	0	NULL	Six	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we summarise the pattern of expression of certain genes involved in the eye network that have been isolated in planarians , such as Otx , Pax-6 , Six , Rax and opsin .
	manualset3
85758	7	398468	14	13	NULL	0	NULL	Rax	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we summarise the pattern of expression of certain genes involved in the eye network that have been isolated in planarians , such as Otx , Pax-6 , Six , Rax and opsin .
	manualset3
85759	8	398468	14	13	NULL	0	NULL	opsin	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we summarise the pattern of expression of certain genes involved in the eye network that have been isolated in planarians , such as Otx , Pax-6 , Six , Rax and opsin .
	manualset3
85760	1	398469	14	13	NULL	0	NULL	 immunogenicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we tested the immunogenicity and protective effectiveness of attenuated F18ac ( + ) non-ETEC vaccine candidate strain against challenge infection with F4ac ( + ) ETEC strain by quantitative phenotypic analysis of small intestinal leukocyte subsets in weaned pigs .
	manualset3
85761	2	398469	14	13	NULL	0	NULL	protective effectiveness 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we tested the immunogenicity and protective effectiveness of attenuated F18ac ( + ) non-ETEC vaccine candidate strain against challenge infection with F4ac ( + ) ETEC strain by quantitative phenotypic analysis of small intestinal leukocyte subsets in weaned pigs .
	manualset3
85762	3	398469	14	13	NULL	0	NULL	attenuated F18ac ( + ) non-ETEC vaccine candidate strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we tested the immunogenicity and protective effectiveness of attenuated F18ac ( + ) non-ETEC vaccine candidate strain against challenge infection with F4ac ( + ) ETEC strain by quantitative phenotypic analysis of small intestinal leukocyte subsets in weaned pigs .
	manualset3
85763	4	398469	14	13	NULL	0	NULL	challenge infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we tested the immunogenicity and protective effectiveness of attenuated F18ac ( + ) non-ETEC vaccine candidate strain against challenge infection with F4ac ( + ) ETEC strain by quantitative phenotypic analysis of small intestinal leukocyte subsets in weaned pigs .
	manualset3
85764	5	398469	14	13	NULL	0	NULL	F4ac ( + ) ETEC strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we tested the immunogenicity and protective effectiveness of attenuated F18ac ( + ) non-ETEC vaccine candidate strain against challenge infection with F4ac ( + ) ETEC strain by quantitative phenotypic analysis of small intestinal leukocyte subsets in weaned pigs .
	manualset3
85765	6	398469	14	13	NULL	0	NULL	quantitative phenotypic analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we tested the immunogenicity and protective effectiveness of attenuated F18ac ( + ) non-ETEC vaccine candidate strain against challenge infection with F4ac ( + ) ETEC strain by quantitative phenotypic analysis of small intestinal leukocyte subsets in weaned pigs .
	manualset3
85766	7	398469	14	13	NULL	0	NULL	small intestinal leukocyte subsets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we tested the immunogenicity and protective effectiveness of attenuated F18ac ( + ) non-ETEC vaccine candidate strain against challenge infection with F4ac ( + ) ETEC strain by quantitative phenotypic analysis of small intestinal leukocyte subsets in weaned pigs .
	manualset3
85767	8	398469	14	13	NULL	0	NULL	weaned pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we tested the immunogenicity and protective effectiveness of attenuated F18ac ( + ) non-ETEC vaccine candidate strain against challenge infection with F4ac ( + ) ETEC strain by quantitative phenotypic analysis of small intestinal leukocyte subsets in weaned pigs .
	manualset3
85768	1	398470	14	13	NULL	0	NULL	 Synthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Synthesis of porcine brain natriuretic peptide ( BNP-26 ) and an analog ) .
	manualset3
85769	2	398470	14	13	NULL	NULL	NULL	porcine brain natriuretic peptide ( BNP-26 )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Synthesis of porcine brain natriuretic peptide ( BNP-26 ) and an analog ) .
	manualset3
85770	3	398470	14	13	NULL	NULL	NULL	analog	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Synthesis of porcine brain natriuretic peptide ( BNP-26 ) and an analog ) .
	manualset3
85777	1	398472	14	13	NULL	NULL	NULL	fiber taper waveguide	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we use a fiber taper waveguide to perform direct optical spectroscopy of a system consisting of a quantum dot embedded in a microdisk .
	manualset3
85778	2	398472	14	13	NULL	NULL	NULL	optical spectroscopy	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we use a fiber taper waveguide to perform direct optical spectroscopy of a system consisting of a quantum dot embedded in a microdisk .
	manualset3
85779	4	398472	14	13	NULL	NULL	NULL	microdisk 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we use a fiber taper waveguide to perform direct optical spectroscopy of a system consisting of a quantum dot embedded in a microdisk .
	manualset3
86134	3	398472	14	13	NULL	0	NULL	quantum dot \t	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we use a fiber taper waveguide to perform direct optical spectroscopy of a system consisting of a quantum dot embedded in a microdisk .
	manualset3
85780	1	398473	14	13	NULL	NULL	NULL	genetic recapture data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we used genetic recapture data to quantify male site fidelity at a colony of Antarctic fur seals where an aerial walkway provides unprecedented access and individual positions are determined daily to 1 m accuracy .
	manualset3
85781	2	398473	14	13	NULL	0	NULL	male site fidelity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we used genetic recapture data to quantify male site fidelity at a colony of Antarctic fur seals where an aerial walkway provides unprecedented access and individual positions are determined daily to 1 m accuracy .
	manualset3
85782	3	398473	14	13	NULL	0	NULL	 colony of Antarctic fur seals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we used genetic recapture data to quantify male site fidelity at a colony of Antarctic fur seals where an aerial walkway provides unprecedented access and individual positions are determined daily to 1 m accuracy .
	manualset3
85783	4	398473	14	13	NULL	NULL	NULL	 aerial walkway	Thing												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we used genetic recapture data to quantify male site fidelity at a colony of Antarctic fur seals where an aerial walkway provides unprecedented access and individual positions are determined daily to 1 m accuracy .
	manualset3
85784	5	398473	14	13	NULL	0	NULL	daily	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we used genetic recapture data to quantify male site fidelity at a colony of Antarctic fur seals where an aerial walkway provides unprecedented access and individual positions are determined daily to 1 m accuracy .
	manualset3
85785	6	398473	14	13	NULL	NULL	NULL	1 m 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we used genetic recapture data to quantify male site fidelity at a colony of Antarctic fur seals where an aerial walkway provides unprecedented access and individual positions are determined daily to 1 m accuracy .
	manualset3
85786	1	398474	14	13	NULL	0	NULL	intrahippocampal microinfusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we used intrahippocampal microinfusion of BDNF to analyze its effects on functional and structural synaptic plasticity induced by subsequent mossy fiber HFS sufficient to induce LTP in adult rats , in vivo .
	manualset3
85787	2	398474	14	13	NULL	0	NULL	BDNF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we used intrahippocampal microinfusion of BDNF to analyze its effects on functional and structural synaptic plasticity induced by subsequent mossy fiber HFS sufficient to induce LTP in adult rats , in vivo .
	manualset3
85788	3	398474	14	13	NULL	0	NULL	functional and structural synaptic plasticity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we used intrahippocampal microinfusion of BDNF to analyze its effects on functional and structural synaptic plasticity induced by subsequent mossy fiber HFS sufficient to induce LTP in adult rats , in vivo .
	manualset3
85789	4	398474	14	13	NULL	0	NULL	mossy fiber	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we used intrahippocampal microinfusion of BDNF to analyze its effects on functional and structural synaptic plasticity induced by subsequent mossy fiber HFS sufficient to induce LTP in adult rats , in vivo .
	manualset3
85790	5	398474	14	13	NULL	0	NULL	HFS	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we used intrahippocampal microinfusion of BDNF to analyze its effects on functional and structural synaptic plasticity induced by subsequent mossy fiber HFS sufficient to induce LTP in adult rats , in vivo .
	manualset3
85791	6	398474	14	13	NULL	0	NULL	LTP	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we used intrahippocampal microinfusion of BDNF to analyze its effects on functional and structural synaptic plasticity induced by subsequent mossy fiber HFS sufficient to induce LTP in adult rats , in vivo .
	manualset3
85792	7	398474	14	13	NULL	0	NULL	adult rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we used intrahippocampal microinfusion of BDNF to analyze its effects on functional and structural synaptic plasticity induced by subsequent mossy fiber HFS sufficient to induce LTP in adult rats , in vivo .
	manualset3
85793	1	398475	14	13	NULL	0	NULL	linkage group selection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we used linkage group selection and Solexa whole-genome resequencing to investigate the genetic basis of resistance to component drugs of ACTs .
	manualset3
85794	2	398475	14	13	NULL	0	NULL	Solexa whole-genome resequencing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we used linkage group selection and Solexa whole-genome resequencing to investigate the genetic basis of resistance to component drugs of ACTs .
	manualset3
85795	3	398475	14	13	NULL	0	NULL	genetic basis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we used linkage group selection and Solexa whole-genome resequencing to investigate the genetic basis of resistance to component drugs of ACTs .
	manualset3
85796	4	398475	14	13	NULL	0	NULL	resistance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we used linkage group selection and Solexa whole-genome resequencing to investigate the genetic basis of resistance to component drugs of ACTs .
	manualset3
85797	5	398475	14	13	NULL	0	NULL	component drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we used linkage group selection and Solexa whole-genome resequencing to investigate the genetic basis of resistance to component drugs of ACTs .
	manualset3
85798	6	398475	14	13	NULL	0	NULL	ACTs	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we used linkage group selection and Solexa whole-genome resequencing to investigate the genetic basis of resistance to component drugs of ACTs .
	manualset3
85799	1	398476	14	13	NULL	0	NULL	Hereditary angioedema ( HAE )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hereditary angioedema ( HAE ) is a rare disorder characterized by recurrent attacks of swelling that may involve multiple anatomical locations .
	manualset3
85800	3	398476	14	13	NULL	0	NULL	recurrent attacks of swelling 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hereditary angioedema ( HAE ) is a rare disorder characterized by recurrent attacks of swelling that may involve multiple anatomical locations .
	manualset3
85801	2	398476	14	13	NULL	0	NULL	 rare disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hereditary angioedema ( HAE ) is a rare disorder characterized by recurrent attacks of swelling that may involve multiple anatomical locations .
	manualset3
85802	4	398476	14	13	NULL	0	NULL	multiple anatomical locations	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Hereditary angioedema ( HAE ) is a rare disorder characterized by recurrent attacks of swelling that may involve multiple anatomical locations .
	manualset3
85803	1	398477	14	13	NULL	0	NULL	Hereditary inclusion body myopathy ( HIBM )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hereditary inclusion body myopathy ( HIBM ) is a young-adult onset autosomal recessive disorder caused by a hypomorphic rate limiting enzyme of sialic acid biosynthesis .
	manualset3
85804	2	398477	14	13	NULL	0	NULL	young-adult onset autosomal recessive disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hereditary inclusion body myopathy ( HIBM ) is a young-adult onset autosomal recessive disorder caused by a hypomorphic rate limiting enzyme of sialic acid biosynthesis .
	manualset3
85805	3	398477	14	13	NULL	0	NULL	hypomorphic rate limiting enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hereditary inclusion body myopathy ( HIBM ) is a young-adult onset autosomal recessive disorder caused by a hypomorphic rate limiting enzyme of sialic acid biosynthesis .
	manualset3
85806	4	398477	14	13	NULL	0	NULL	sialic acid biosynthesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hereditary inclusion body myopathy ( HIBM ) is a young-adult onset autosomal recessive disorder caused by a hypomorphic rate limiting enzyme of sialic acid biosynthesis .
	manualset3
85807	1	398478	14	13	NULL	0	NULL	Hereditary nonpolyposis colorectal cancer ( HNPCC )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hereditary nonpolyposis colorectal cancer ( HNPCC ) is a major cancer susceptibility syndrome known to be caused by the inheritance of mutations in DNA mismatch repair genes , such as hMSH2 , hMLH1 , hPMS1 and hPMS2 .
	manualset3
85808	2	398478	14	13	NULL	0	NULL	major cancer susceptibility syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hereditary nonpolyposis colorectal cancer ( HNPCC ) is a major cancer susceptibility syndrome known to be caused by the inheritance of mutations in DNA mismatch repair genes , such as hMSH2 , hMLH1 , hPMS1 and hPMS2 .
	manualset3
85809	3	398478	14	13	NULL	0	NULL	inheritance of mutations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hereditary nonpolyposis colorectal cancer ( HNPCC ) is a major cancer susceptibility syndrome known to be caused by the inheritance of mutations in DNA mismatch repair genes , such as hMSH2 , hMLH1 , hPMS1 and hPMS2 .
	manualset3
85810	4	398478	14	13	NULL	0	NULL	DNA mismatch repair genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hereditary nonpolyposis colorectal cancer ( HNPCC ) is a major cancer susceptibility syndrome known to be caused by the inheritance of mutations in DNA mismatch repair genes , such as hMSH2 , hMLH1 , hPMS1 and hPMS2 .
	manualset3
85811	5	398478	14	13	NULL	0	NULL	hMSH2	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Hereditary nonpolyposis colorectal cancer ( HNPCC ) is a major cancer susceptibility syndrome known to be caused by the inheritance of mutations in DNA mismatch repair genes , such as hMSH2 , hMLH1 , hPMS1 and hPMS2 .
	manualset3
85812	6	398478	14	13	NULL	0	NULL	hMLH1 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Hereditary nonpolyposis colorectal cancer ( HNPCC ) is a major cancer susceptibility syndrome known to be caused by the inheritance of mutations in DNA mismatch repair genes , such as hMSH2 , hMLH1 , hPMS1 and hPMS2 .
	manualset3
85813	7	398478	14	13	NULL	0	NULL	hPMS1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Hereditary nonpolyposis colorectal cancer ( HNPCC ) is a major cancer susceptibility syndrome known to be caused by the inheritance of mutations in DNA mismatch repair genes , such as hMSH2 , hMLH1 , hPMS1 and hPMS2 .
	manualset3
85814	8	398478	14	13	NULL	0	NULL	hPMS2 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Hereditary nonpolyposis colorectal cancer ( HNPCC ) is a major cancer susceptibility syndrome known to be caused by the inheritance of mutations in DNA mismatch repair genes , such as hMSH2 , hMLH1 , hPMS1 and hPMS2 .
	manualset3
85815	1	398479	14	13	NULL	0	NULL	Hereditary spherocytosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hereditary spherocytosis and elliptocytosis erythrocytes show a normal transbilayer phospholipid distribution .
	manualset3
85816	2	398479	14	13	NULL	0	NULL	elliptocytosis erythrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Hereditary spherocytosis and elliptocytosis erythrocytes show a normal transbilayer phospholipid distribution .
	manualset3
85817	3	398479	14	13	NULL	0	NULL	normal transbilayer phospholipid distribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hereditary spherocytosis and elliptocytosis erythrocytes show a normal transbilayer phospholipid distribution .
	manualset3
85823	1	398481	14	13	NULL	NULL	NULL	Synthesis of quinolines	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Synthesis of quinolines from safrole ) .
	manualset3
85824	2	398481	14	13	NULL	0	NULL	safrole	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Synthesis of quinolines from safrole ) .
	manualset3
85830	1	398483	14	13	NULL	0	NULL	hispolon	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Herein , we report our findings that hispolon inhibited breast and bladder cancer cell growth , regardless of p53 status .
	manualset3
85831	2	398483	14	13	NULL	0	NULL	 breast and bladder cancer cell growth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Herein , we report our findings that hispolon inhibited breast and bladder cancer cell growth , regardless of p53 status .
	manualset3
85832	3	398483	14	13	NULL	0	NULL	p53	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Herein , we report our findings that hispolon inhibited breast and bladder cancer cell growth , regardless of p53 status .
	manualset3
85833	1	398484	14	13	NULL	NULL	NULL	epigenetic findings	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Herein , we review relevant epigenetic findings associated with psoriasis , and provide clues and directions for further studies in this field .
	manualset3
85834	2	398484	14	13	NULL	NULL	NULL	psoriasis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Herein , we review relevant epigenetic findings associated with psoriasis , and provide clues and directions for further studies in this field .
	manualset3
86146	3	398484	14	13	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Herein , we review relevant epigenetic findings associated with psoriasis , and provide clues and directions for further studies in this field .
	manualset3
85836	1	398485	14	13	NULL	0	NULL	SrTiO ( 3 ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Herein we show that metallic interfaces can be realized in SrTiO ( 3 ) - based heterostructures with various insulating overlayers of amorphous LaAlO ( 3 ) , SrTiO ( 3 ) , and yttria-stabilized zirconia films .
	manualset3
85837	2	398485	14	13	NULL	0	NULL	 amorphous LaAlO ( 3 ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Herein we show that metallic interfaces can be realized in SrTiO ( 3 ) - based heterostructures with various insulating overlayers of amorphous LaAlO ( 3 ) , SrTiO ( 3 ) , and yttria-stabilized zirconia films .
	manualset3
85838	3	398485	14	13	NULL	0	NULL	SrTiO ( 3 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Herein we show that metallic interfaces can be realized in SrTiO ( 3 ) - based heterostructures with various insulating overlayers of amorphous LaAlO ( 3 ) , SrTiO ( 3 ) , and yttria-stabilized zirconia films .
	manualset3
85839	4	398485	14	13	NULL	NULL	NULL	yttria-stabilized zirconia films	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Herein we show that metallic interfaces can be realized in SrTiO ( 3 ) - based heterostructures with various insulating overlayers of amorphous LaAlO ( 3 ) , SrTiO ( 3 ) , and yttria-stabilized zirconia films .
	manualset3
85846	1	398487	14	13	NULL	NULL	NULL	Herniography	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Herniography , computed tomography ( CT ) , and magnetic resonance ( MR ) imaging are also helpful in diagnosis .
	manualset3
85847	2	398487	14	13	NULL	NULL	NULL	computed tomography ( CT ) 	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Herniography , computed tomography ( CT ) , and magnetic resonance ( MR ) imaging are also helpful in diagnosis .
	manualset3
85848	3	398487	14	13	NULL	NULL	NULL	magnetic resonance ( MR ) imaging	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Herniography , computed tomography ( CT ) , and magnetic resonance ( MR ) imaging are also helpful in diagnosis .
	manualset3
85849	4	398487	14	13	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Herniography , computed tomography ( CT ) , and magnetic resonance ( MR ) imaging are also helpful in diagnosis .
	manualset3
85850	1	398488	14	13	NULL	NULL	NULL	Systems for financing and delivery 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Systems for financing and delivery of dental care ) .
	manualset3
85851	2	398488	14	13	NULL	0	NULL	dental care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Systems for financing and delivery of dental care ) .
	manualset3
85852	1	398489	14	13	NULL	NULL	NULL	Herpes simplex virus type 1 infection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Herpes simplex virus type 1 infection activates the Epstein-Barr virus replicative cycle via a CREB-dependent mechanism .
	manualset3
85853	2	398489	14	13	NULL	0	NULL	Epstein-Barr virus replicative cycle	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Herpes simplex virus type 1 infection activates the Epstein-Barr virus replicative cycle via a CREB-dependent mechanism .
	manualset3
85854	3	398489	14	13	NULL	0	NULL	 CREB-dependent mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Herpes simplex virus type 1 infection activates the Epstein-Barr virus replicative cycle via a CREB-dependent mechanism .
	manualset3
85855	1	398490	14	13	NULL	0	NULL	Herpes simplex virus type 2 meningitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Herpes simplex virus type 2 meningitis and associated genital lesions in a three-year-old child .
	manualset3
85856	2	398490	14	13	NULL	0	NULL	genital lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Herpes simplex virus type 2 meningitis and associated genital lesions in a three-year-old child .
	manualset3
85857	3	398490	14	13	NULL	0	NULL	three-year-old child	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Herpes simplex virus type 2 meningitis and associated genital lesions in a three-year-old child .
	manualset3
85858	1	398491	14	13	NULL	0	NULL	Heteroaromatic synthesis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Heteroaromatic synthesis via olefin cross-metathesis : entry to polysubstituted pyridines .
	manualset3
85859	2	398491	14	13	NULL	0	NULL	olefin cross-metathesis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Heteroaromatic synthesis via olefin cross-metathesis : entry to polysubstituted pyridines .
	manualset3
85861	3	398491	14	13	NULL	0	NULL	polysubstituted pyridines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Heteroaromatic synthesis via olefin cross-metathesis : entry to polysubstituted pyridines .
	manualset3
85862	1	398492	14	13	NULL	0	NULL	Heterochromatisation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heterochromatisation as a change of chromosome cycle .
	manualset3
85863	2	398492	14	13	NULL	0	NULL	chromosome cycle	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heterochromatisation as a change of chromosome cycle .
	manualset3
85864	1	398493	14	13	NULL	0	NULL	Heteroduplex analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Heteroduplex analysis and restriction endonuclease mapping experiments indicate that the LpE family is more closely related to the B-C than the A-D family of early histone genes .
	manualset3
85865	2	398493	14	13	NULL	0	NULL	restriction endonuclease mapping experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Heteroduplex analysis and restriction endonuclease mapping experiments indicate that the LpE family is more closely related to the B-C than the A-D family of early histone genes .
	manualset3
85866	3	398493	14	13	NULL	0	NULL	LpE family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Heteroduplex analysis and restriction endonuclease mapping experiments indicate that the LpE family is more closely related to the B-C than the A-D family of early histone genes .
	manualset3
85867	4	398493	14	13	NULL	0	NULL	B-C family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Heteroduplex analysis and restriction endonuclease mapping experiments indicate that the LpE family is more closely related to the B-C than the A-D family of early histone genes .
	manualset3
85868	5	398493	14	13	NULL	0	NULL	A-D family of early histone genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Heteroduplex analysis and restriction endonuclease mapping experiments indicate that the LpE family is more closely related to the B-C than the A-D family of early histone genes .
	manualset3
85873	1	398495	14	13	NULL	0	NULL	Heterogeneous nuclear RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Heterogeneous nuclear RNA is normally complexed with a specific set of proteins , forming ribonucleoprotein particles termed hnRNP .
	manualset3
85874	2	398495	14	13	NULL	0	NULL	specific set of proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Heterogeneous nuclear RNA is normally complexed with a specific set of proteins , forming ribonucleoprotein particles termed hnRNP .
	manualset3
85875	3	398495	14	13	NULL	0	NULL	ribonucleoprotein particles	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Heterogeneous nuclear RNA is normally complexed with a specific set of proteins , forming ribonucleoprotein particles termed hnRNP .
	manualset3
85876	4	398495	14	13	NULL	0	NULL	hnRNP	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Heterogeneous nuclear RNA is normally complexed with a specific set of proteins , forming ribonucleoprotein particles termed hnRNP .
	manualset3
85877	1	398496	14	13	NULL	0	NULL	Heterogeneous ribonucleoprotein C	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Heterogeneous ribonucleoprotein C displays a repressor activity mediated by T-cell intracellular antigen-1-related / like protein to modulate Fas exon 6 splicing through a mechanism involving Hu antigen R .
	manualset3
85878	2	398496	14	13	NULL	0	NULL	repressor activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heterogeneous ribonucleoprotein C displays a repressor activity mediated by T-cell intracellular antigen-1-related / like protein to modulate Fas exon 6 splicing through a mechanism involving Hu antigen R .
	manualset3
85879	3	398496	14	13	NULL	0	NULL	T-cell intracellular antigen-1-related / like protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Heterogeneous ribonucleoprotein C displays a repressor activity mediated by T-cell intracellular antigen-1-related / like protein to modulate Fas exon 6 splicing through a mechanism involving Hu antigen R .
	manualset3
85880	4	398496	14	13	NULL	0	NULL	Fas exon 6 splicing	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heterogeneous ribonucleoprotein C displays a repressor activity mediated by T-cell intracellular antigen-1-related / like protein to modulate Fas exon 6 splicing through a mechanism involving Hu antigen R .
	manualset3
85881	5	398496	14	13	NULL	0	NULL	Hu antigen R	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Heterogeneous ribonucleoprotein C displays a repressor activity mediated by T-cell intracellular antigen-1-related / like protein to modulate Fas exon 6 splicing through a mechanism involving Hu antigen R .
	manualset3
85882	1	398497	14	13	NULL	0	NULL	Heterokaryosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heterokaryosis in Fusarium oxysporum f. sp .
	manualset3
85883	2	398497	14	13	NULL	0	NULL	Fusarium oxysporum f. sp	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Heterokaryosis in Fusarium oxysporum f. sp .
	manualset3
85884	1	398498	14	13	NULL	0	NULL	Heterologous expression of lipoprotein-associated phospholipase A2 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heterologous expression of lipoprotein-associated phospholipase A2 in different expression systems .
	manualset3
86140	2	398498	14	13	NULL	0	NULL	 different expression systems	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Heterologous expression of lipoprotein-associated phospholipase A2 in different expression systems .
	manualset3
85885	1	398499	14	13	NULL	0	NULL	Heterooligomerization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heterooligomerization of human dopamine receptor 2 and somatostatin receptor 2 Co-immunoprecipitation and fluorescence resonance energy transfer analysis .
	manualset3
85886	2	398499	14	13	NULL	0	NULL	human dopamine receptor 2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Heterooligomerization of human dopamine receptor 2 and somatostatin receptor 2 Co-immunoprecipitation and fluorescence resonance energy transfer analysis .
	manualset3
85887	3	398499	14	13	NULL	0	NULL	somatostatin receptor 2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Heterooligomerization of human dopamine receptor 2 and somatostatin receptor 2 Co-immunoprecipitation and fluorescence resonance energy transfer analysis .
	manualset3
85888	4	398499	14	13	NULL	0	NULL	Co-immunoprecipitation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Heterooligomerization of human dopamine receptor 2 and somatostatin receptor 2 Co-immunoprecipitation and fluorescence resonance energy transfer analysis .
	manualset3
85889	5	398499	14	13	NULL	0	NULL	fluorescence resonance energy transfer analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Heterooligomerization of human dopamine receptor 2 and somatostatin receptor 2 Co-immunoprecipitation and fluorescence resonance energy transfer analysis .
	manualset3
85890	1	398500	14	13	NULL	0	NULL	Heterophile antibodies	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Heterophile antibodies and the diagnosis of Rocky Mountain spotted fever .
	manualset3
85891	2	398500	14	13	NULL	NULL	NULL	diagnosis 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Heterophile antibodies and the diagnosis of Rocky Mountain spotted fever .
	manualset3
85894	3	398500	14	13	NULL	0	NULL	Rocky Mountain spotted fever	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Heterophile antibodies and the diagnosis of Rocky Mountain spotted fever .
	manualset3
85895	1	398501	14	13	NULL	NULL	NULL	Heterotopic bone	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Heterotopic bone in the abdominal wall due to metastatic transitional cell carcinoma in a dog .
	manualset3
85896	2	398501	14	13	NULL	0	NULL	abdominal wall 	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Heterotopic bone in the abdominal wall due to metastatic transitional cell carcinoma in a dog .
	manualset3
85897	3	398501	14	13	NULL	0	NULL	metastatic transitional cell carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Heterotopic bone in the abdominal wall due to metastatic transitional cell carcinoma in a dog .
	manualset3
85898	4	398501	14	13	NULL	0	NULL	dog	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Heterotopic bone in the abdominal wall due to metastatic transitional cell carcinoma in a dog .
	manualset3
85899	1	398502	14	13	NULL	0	NULL	Hexafluorocyclobutene ( HFCB )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hexafluorocyclobutene ( HFCB ) , a reactive organohalogen gas , causes overwhelming pulmonary oedema .
	manualset3
85900	2	398502	14	13	NULL	0	NULL	reactive organohalogen gas	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hexafluorocyclobutene ( HFCB ) , a reactive organohalogen gas , causes overwhelming pulmonary oedema .
	manualset3
85901	3	398502	14	13	NULL	0	NULL	overwhelming pulmonary oedema	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hexafluorocyclobutene ( HFCB ) , a reactive organohalogen gas , causes overwhelming pulmonary oedema .
	manualset3
85902	1	398503	14	13	NULL	0	NULL	T cell non-Hodgkin 's lymphoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( T cell non-Hodgkin 's lymphoma of the external auditory canal ) .
	manualset3
85903	2	398503	14	13	NULL	0	NULL	external auditory canal 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( T cell non-Hodgkin 's lymphoma of the external auditory canal ) .
	manualset3
85904	1	398504	14	13	NULL	0	NULL	Hexokinase ( EC 2.7.1.1 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hexokinase ( EC 2.7.1.1 ) , NAD-dependent malate dehydrogenase ( EC 1.1.1.37 ) , malic enzyme ( EC 1.1.1.40 ) , lactate dehydrogenase ( EC 1.1.1.27 ) , alcohol dehydrogenase ( EC 1.1.1.1 ) and succinate dehydrogenase ( EC 1.3.99.1 ) were not detectable .
	manualset3
85905	2	398504	14	13	NULL	0	NULL	NAD-dependent malate dehydrogenase ( EC 1.1.1.37 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hexokinase ( EC 2.7.1.1 ) , NAD-dependent malate dehydrogenase ( EC 1.1.1.37 ) , malic enzyme ( EC 1.1.1.40 ) , lactate dehydrogenase ( EC 1.1.1.27 ) , alcohol dehydrogenase ( EC 1.1.1.1 ) and succinate dehydrogenase ( EC 1.3.99.1 ) were not detectable .
	manualset3
85906	3	398504	14	13	NULL	0	NULL	malic enzyme ( EC 1.1.1.40 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hexokinase ( EC 2.7.1.1 ) , NAD-dependent malate dehydrogenase ( EC 1.1.1.37 ) , malic enzyme ( EC 1.1.1.40 ) , lactate dehydrogenase ( EC 1.1.1.27 ) , alcohol dehydrogenase ( EC 1.1.1.1 ) and succinate dehydrogenase ( EC 1.3.99.1 ) were not detectable .
	manualset3
85907	4	398504	14	13	NULL	0	NULL	lactate dehydrogenase ( EC 1.1.1.27 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hexokinase ( EC 2.7.1.1 ) , NAD-dependent malate dehydrogenase ( EC 1.1.1.37 ) , malic enzyme ( EC 1.1.1.40 ) , lactate dehydrogenase ( EC 1.1.1.27 ) , alcohol dehydrogenase ( EC 1.1.1.1 ) and succinate dehydrogenase ( EC 1.3.99.1 ) were not detectable .
	manualset3
85908	5	398504	14	13	NULL	0	NULL	alcohol dehydrogenase ( EC 1.1.1.1 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hexokinase ( EC 2.7.1.1 ) , NAD-dependent malate dehydrogenase ( EC 1.1.1.37 ) , malic enzyme ( EC 1.1.1.40 ) , lactate dehydrogenase ( EC 1.1.1.27 ) , alcohol dehydrogenase ( EC 1.1.1.1 ) and succinate dehydrogenase ( EC 1.3.99.1 ) were not detectable .
	manualset3
85909	6	398504	14	13	NULL	0	NULL	succinate dehydrogenase ( EC 1.3.99.1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hexokinase ( EC 2.7.1.1 ) , NAD-dependent malate dehydrogenase ( EC 1.1.1.37 ) , malic enzyme ( EC 1.1.1.40 ) , lactate dehydrogenase ( EC 1.1.1.27 ) , alcohol dehydrogenase ( EC 1.1.1.1 ) and succinate dehydrogenase ( EC 1.3.99.1 ) were not detectable .
	manualset3
85910	1	398505	14	13	NULL	0	NULL	Hexose-monophosphate shunt ( HMS ) activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hexose-monophosphate shunt ( HMS ) activity , myelo-peroxidase - ( MPO ) - mediated iodination and random mobility in human polymorphonuclear leukocytes ( PMNs ) were studied in the presence of lignocaine .
	manualset3
85911	2	398505	14	13	NULL	0	NULL	myelo-peroxidase - ( MPO ) - mediated iodination	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hexose-monophosphate shunt ( HMS ) activity , myelo-peroxidase - ( MPO ) - mediated iodination and random mobility in human polymorphonuclear leukocytes ( PMNs ) were studied in the presence of lignocaine .
	manualset3
85912	3	398505	14	13	NULL	NULL	NULL	random mobility 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hexose-monophosphate shunt ( HMS ) activity , myelo-peroxidase - ( MPO ) - mediated iodination and random mobility in human polymorphonuclear leukocytes ( PMNs ) were studied in the presence of lignocaine .
	manualset3
85913	4	398505	14	13	NULL	0	NULL	human polymorphonuclear leukocytes ( PMNs )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Hexose-monophosphate shunt ( HMS ) activity , myelo-peroxidase - ( MPO ) - mediated iodination and random mobility in human polymorphonuclear leukocytes ( PMNs ) were studied in the presence of lignocaine .
	manualset3
85914	5	398505	14	13	NULL	0	NULL	lignocaine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Hexose-monophosphate shunt ( HMS ) activity , myelo-peroxidase - ( MPO ) - mediated iodination and random mobility in human polymorphonuclear leukocytes ( PMNs ) were studied in the presence of lignocaine .
	manualset3
85915	1	398506	14	13	NULL	NULL	NULL	Hierarchical clustering of the 17 miRNAs expression profiles	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hierarchical clustering of the 17 miRNAs expression profiles showed that individuals with active TB clustered independently of individuals with LTBI or from healthy controls .
	manualset3
85917	3	398506	14	13	NULL	0	NULL	 individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hierarchical clustering of the 17 miRNAs expression profiles showed that individuals with active TB clustered independently of individuals with LTBI or from healthy controls .
	manualset3
85918	4	398506	14	13	NULL	0	NULL	active TB	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hierarchical clustering of the 17 miRNAs expression profiles showed that individuals with active TB clustered independently of individuals with LTBI or from healthy controls .
	manualset3
85919	5	398506	14	13	NULL	NULL	NULL	individuals with LTBI 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hierarchical clustering of the 17 miRNAs expression profiles showed that individuals with active TB clustered independently of individuals with LTBI or from healthy controls .
	manualset3
85920	6	398506	14	13	NULL	0	NULL	healthy controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hierarchical clustering of the 17 miRNAs expression profiles showed that individuals with active TB clustered independently of individuals with LTBI or from healthy controls .
	manualset3
85921	1	398507	14	13	NULL	0	NULL	High-content screening ( HCS ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	High-content screening ( HCS ) , historically limited to drug-development companies , is now a powerful and affordable technology for academic researchers .
	manualset3
85922	2	398507	14	13	NULL	0	NULL	drug-development companies	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	High-content screening ( HCS ) , historically limited to drug-development companies , is now a powerful and affordable technology for academic researchers .
	manualset3
85923	3	398507	14	13	NULL	NULL	NULL	powerful and affordable technology	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	High-content screening ( HCS ) , historically limited to drug-development companies , is now a powerful and affordable technology for academic researchers .
	manualset3
85924	4	398507	14	13	NULL	0	NULL	academic researchers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	High-content screening ( HCS ) , historically limited to drug-development companies , is now a powerful and affordable technology for academic researchers .
	manualset3
85928	1	398509	14	13	NULL	0	NULL	High-dose intravenous methylprednisolone pulse therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	High-dose intravenous methylprednisolone pulse therapy in systemic lupus erythematosus .
	manualset3
85929	2	398509	14	13	NULL	0	NULL	systemic lupus erythematosus 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	High-dose intravenous methylprednisolone pulse therapy in systemic lupus erythematosus .
	manualset3
85930	1	398510	14	13	NULL	0	NULL	High-flow cardiopulmonary bypass	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	High-flow cardiopulmonary bypass , vasodilating inhalation anesthesia and continuation of Inderal therapy may account for our results .
	manualset3
85931	2	398510	14	13	NULL	0	NULL	vasodilating inhalation anesthesia	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	High-flow cardiopulmonary bypass , vasodilating inhalation anesthesia and continuation of Inderal therapy may account for our results .
	manualset3
85932	3	398510	14	13	NULL	0	NULL	Inderal therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	High-flow cardiopulmonary bypass , vasodilating inhalation anesthesia and continuation of Inderal therapy may account for our results .
	manualset3
85933	1	398511	14	13	NULL	0	NULL	High-passage poorly differentiated cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	High-passage poorly differentiated cells were refractory to PTHRP .
	manualset3
85934	2	398511	14	13	NULL	0	NULL	PTHRP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	High-passage poorly differentiated cells were refractory to PTHRP .
	manualset3
85935	1	398512	14	13	NULL	NULL	NULL	( 2 , 3 , 4 , 4-Tetramethylcyclopentyl ) methyl acetate 	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( 2 , 3 , 4 , 4-Tetramethylcyclopentyl ) methyl acetate , a sex pheromone from the obscure mealybug : first example of a new structural class of monoterpenes .
	manualset3
85936	2	398512	14	13	NULL	NULL	NULL	sex pheromone	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( 2 , 3 , 4 , 4-Tetramethylcyclopentyl ) methyl acetate , a sex pheromone from the obscure mealybug : first example of a new structural class of monoterpenes .
	manualset3
85937	3	398512	14	13	NULL	0	NULL	obscure mealybug	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( 2 , 3 , 4 , 4-Tetramethylcyclopentyl ) methyl acetate , a sex pheromone from the obscure mealybug : first example of a new structural class of monoterpenes .
	manualset3
85938	4	398512	14	13	NULL	NULL	NULL	structural class of monoterpenes 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( 2 , 3 , 4 , 4-Tetramethylcyclopentyl ) methyl acetate , a sex pheromone from the obscure mealybug : first example of a new structural class of monoterpenes .
	manualset3
86012	1	398513	14	13	NULL	0	NULL	Analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Analysis of immune response to Japanese encephalitis virus infection in mice : effect of cyclosporin A on the production of HI antibody and interferon ) .
	manualset3
86013	2	398513	14	13	NULL	0	NULL	immune response to Japanese encephalitis virus infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Analysis of immune response to Japanese encephalitis virus infection in mice : effect of cyclosporin A on the production of HI antibody and interferon ) .
	manualset3
86014	3	398513	14	13	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Analysis of immune response to Japanese encephalitis virus infection in mice : effect of cyclosporin A on the production of HI antibody and interferon ) .
	manualset3
86015	4	398513	14	13	NULL	0	NULL	cyclosporin A	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Analysis of immune response to Japanese encephalitis virus infection in mice : effect of cyclosporin A on the production of HI antibody and interferon ) .
	manualset3
86016	5	398513	14	13	NULL	0	NULL	production of HI antibody	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Analysis of immune response to Japanese encephalitis virus infection in mice : effect of cyclosporin A on the production of HI antibody and interferon ) .
	manualset3
86017	6	398513	14	13	NULL	NULL	NULL	production of interferon 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Analysis of immune response to Japanese encephalitis virus infection in mice : effect of cyclosporin A on the production of HI antibody and interferon ) .
	manualset3
86022	1	398515	14	13	NULL	0	NULL	High-performance liquid chromatographic determination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	High-performance liquid chromatographic determination of lansoprazole and its metabolites in human serum and urine .
	manualset3
86023	2	398515	14	13	NULL	0	NULL	lansoprazole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	High-performance liquid chromatographic determination of lansoprazole and its metabolites in human serum and urine .
	manualset3
86024	3	398515	14	13	NULL	0	NULL	metabolites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	High-performance liquid chromatographic determination of lansoprazole and its metabolites in human serum and urine .
	manualset3
86025	4	398515	14	13	NULL	0	NULL	human serum	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	High-performance liquid chromatographic determination of lansoprazole and its metabolites in human serum and urine .
	manualset3
86026	5	398515	14	13	NULL	0	NULL	urine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	High-performance liquid chromatographic determination of lansoprazole and its metabolites in human serum and urine .
	manualset3
86027	1	398516	14	13	NULL	0	NULL	High-performance liquid chromatographic microdetermination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	High-performance liquid chromatographic microdetermination of indoprofen in human milk .
	manualset3
86029	2	398516	14	13	NULL	0	NULL	indoprofen	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	High-performance liquid chromatographic microdetermination of indoprofen in human milk .
	manualset3
86030	3	398516	14	13	NULL	0	NULL	human milk 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	High-performance liquid chromatographic microdetermination of indoprofen in human milk .
	manualset3
86031	1	398517	14	13	NULL	0	NULL	High-pressure liquid chromatographic assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	High-pressure liquid chromatographic assays of dopamine and its primary metabolites , homovanillic acid and 3 , 4-dihydroxyphenylacetic acid , showed normal findings .
	manualset3
86034	2	398517	14	13	NULL	NULL	NULL	dopamine	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	High-pressure liquid chromatographic assays of dopamine and its primary metabolites , homovanillic acid and 3 , 4-dihydroxyphenylacetic acid , showed normal findings .
	manualset3
86035	3	398517	14	13	NULL	0	NULL	primary metabolites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	High-pressure liquid chromatographic assays of dopamine and its primary metabolites , homovanillic acid and 3 , 4-dihydroxyphenylacetic acid , showed normal findings .
	manualset3
86045	4	398517	14	13	NULL	0	NULL	 homovanillic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	High-pressure liquid chromatographic assays of dopamine and its primary metabolites , homovanillic acid and 3 , 4-dihydroxyphenylacetic acid , showed normal findings .
	manualset3
86046	5	398517	14	13	NULL	0	NULL	3 , 4-dihydroxyphenylacetic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	High-pressure liquid chromatographic assays of dopamine and its primary metabolites , homovanillic acid and 3 , 4-dihydroxyphenylacetic acid , showed normal findings .
	manualset3
86047	6	398517	14	13	NULL	NULL	NULL	normal findings 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	High-pressure liquid chromatographic assays of dopamine and its primary metabolites , homovanillic acid and 3 , 4-dihydroxyphenylacetic acid , showed normal findings .
	manualset3
86049	1	398518	14	13	NULL	0	NULL	High-resolution bone imaging 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	High-resolution bone imaging has made tremendous progress in the recent past .
	manualset3
86055	3	398518	14	13	NULL	NULL	NULL	recent past	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	High-resolution bone imaging has made tremendous progress in the recent past .
	manualset3
86060	1	398519	14	13	NULL	0	NULL	High-resolution subsurface water-ice distributions 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	High-resolution subsurface water-ice distributions on Mars .
	manualset3
86061	2	398519	14	13	NULL	NULL	NULL	Mars	GeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	High-resolution subsurface water-ice distributions on Mars .
	manualset3
86067	1	398521	14	13	NULL	0	NULL	High-sensitivity C-reactive protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	High-sensitivity C-reactive protein , statin therapy , and risks of atrial fibrillation : an exploratory analysis of the JUPITER trial .
	manualset3
86068	2	398521	14	13	NULL	0	NULL	statin therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	High-sensitivity C-reactive protein , statin therapy , and risks of atrial fibrillation : an exploratory analysis of the JUPITER trial .
	manualset3
86069	3	398521	14	13	NULL	0	NULL	 risks of atrial fibrillation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	High-sensitivity C-reactive protein , statin therapy , and risks of atrial fibrillation : an exploratory analysis of the JUPITER trial .
	manualset3
86070	4	398521	14	13	NULL	0	NULL	exploratory analysis of the JUPITER trial	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	High-sensitivity C-reactive protein , statin therapy , and risks of atrial fibrillation : an exploratory analysis of the JUPITER trial .
	manualset3
86080	1	398524	14	13	NULL	NULL	NULL	simultaneous three-dimensional T ( 2 )	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	High accuracy for simultaneous three-dimensional T ( 2 ) and apparent diffusion coefficient measurements are demonstrated , while also providing morphologic three-dimensional images without blurring or distortion in reasonable scan times .
	manualset3
86081	2	398524	14	13	NULL	0	NULL	apparent diffusion coefficient measurements	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	High accuracy for simultaneous three-dimensional T ( 2 ) and apparent diffusion coefficient measurements are demonstrated , while also providing morphologic three-dimensional images without blurring or distortion in reasonable scan times .
	manualset3
86082	3	398524	14	13	NULL	NULL	NULL	morphologic three-dimensional images	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	High accuracy for simultaneous three-dimensional T ( 2 ) and apparent diffusion coefficient measurements are demonstrated , while also providing morphologic three-dimensional images without blurring or distortion in reasonable scan times .
	manualset3
86083	4	398524	14	13	NULL	NULL	NULL	reasonable scan times 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	High accuracy for simultaneous three-dimensional T ( 2 ) and apparent diffusion coefficient measurements are demonstrated , while also providing morphologic three-dimensional images without blurring or distortion in reasonable scan times .
	manualset3
86084	1	398525	14	13	NULL	0	NULL	High content cellular immune profiling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	High content cellular immune profiling reveals differences between rhesus monkeys and men .
	manualset3
86085	2	398525	14	13	NULL	0	NULL	rhesus monkeys	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	High content cellular immune profiling reveals differences between rhesus monkeys and men .
	manualset3
86086	3	398525	14	13	NULL	0	NULL	men	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	High content cellular immune profiling reveals differences between rhesus monkeys and men .
	manualset3
86087	1	398526	14	13	NULL	0	NULL	High deletion frequency	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	High deletion frequency of the complete AZFa sequence in men with Sertoli-cell-only syndrome .
	manualset3
86088	2	398526	14	13	NULL	0	NULL	complete AZFa sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	High deletion frequency of the complete AZFa sequence in men with Sertoli-cell-only syndrome .
	manualset3
86089	3	398526	14	13	NULL	NULL	NULL	men	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	High deletion frequency of the complete AZFa sequence in men with Sertoli-cell-only syndrome .
	manualset3
86090	4	398526	14	13	NULL	0	NULL	Sertoli-cell-only syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	High deletion frequency of the complete AZFa sequence in men with Sertoli-cell-only syndrome .
	manualset3
86091	1	398527	14	13	NULL	0	NULL	High density lipoprotein deficiency 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	High density lipoprotein deficiency and foam cell accumulation in mice with targeted disruption of ATP-binding cassette transporter-1 .
	manualset3
86092	2	398527	14	13	NULL	0	NULL	foam cell accumulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	High density lipoprotein deficiency and foam cell accumulation in mice with targeted disruption of ATP-binding cassette transporter-1 .
	manualset3
86093	3	398527	14	13	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	High density lipoprotein deficiency and foam cell accumulation in mice with targeted disruption of ATP-binding cassette transporter-1 .
	manualset3
86094	4	398527	14	13	NULL	0	NULL	ATP-binding cassette transporter-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	High density lipoprotein deficiency and foam cell accumulation in mice with targeted disruption of ATP-binding cassette transporter-1 .
	manualset3
86095	1	398528	14	13	NULL	NULL	NULL	High doses of myelosuppressive chemotherapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	High doses of myelosuppressive chemotherapy or radiation have been used in preparative regimens with the goal of preventing graft rejection and eradicating malignancy .
	manualset3
86096	2	398528	14	13	NULL	0	NULL	radiation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	High doses of myelosuppressive chemotherapy or radiation have been used in preparative regimens with the goal of preventing graft rejection and eradicating malignancy .
	manualset3
86097	3	398528	14	13	NULL	0	NULL	preparative regimens	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	High doses of myelosuppressive chemotherapy or radiation have been used in preparative regimens with the goal of preventing graft rejection and eradicating malignancy .
	manualset3
86099	4	398528	14	13	NULL	0	NULL	graft rejection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	High doses of myelosuppressive chemotherapy or radiation have been used in preparative regimens with the goal of preventing graft rejection and eradicating malignancy .
	manualset3
86101	5	398528	14	13	NULL	0	NULL	malignancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	High doses of myelosuppressive chemotherapy or radiation have been used in preparative regimens with the goal of preventing graft rejection and eradicating malignancy .
	manualset3
86141	1	398530	14	13	NULL	NULL	NULL	LEGAL RULINGS 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( THE RIGHT TO DECREE LEGAL RULINGS FOR PLANTS NEEDING SUPERVISION .
	manualset3
86142	2	398530	14	13	NULL	NULL	NULL	PLANTS	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( THE RIGHT TO DECREE LEGAL RULINGS FOR PLANTS NEEDING SUPERVISION .
	manualset3
86354	1	398531	13	NULL	NULL	0	NULL	High field T2-weighted sequences	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	High field T2-weighted sequences disclosed hypersignal bilateral and symmetrically located exclusively at substantia nigra ( 3 cases ) , exclusively at globus pallidus ( 1case ) and simultaneously at substantia nigra , globus pallidus and nigro-strital interconnections ( 1case ) .
	manualset3
86355	2	398531	13	NULL	NULL	0	NULL	substantia nigra	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	High field T2-weighted sequences disclosed hypersignal bilateral and symmetrically located exclusively at substantia nigra ( 3 cases ) , exclusively at globus pallidus ( 1case ) and simultaneously at substantia nigra , globus pallidus and nigro-strital interconnections ( 1case ) .
	manualset3
86356	3	398531	13	NULL	NULL	0	NULL	3 cases	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	High field T2-weighted sequences disclosed hypersignal bilateral and symmetrically located exclusively at substantia nigra ( 3 cases ) , exclusively at globus pallidus ( 1case ) and simultaneously at substantia nigra , globus pallidus and nigro-strital interconnections ( 1case ) .
	manualset3
86357	4	398531	13	NULL	NULL	0	NULL	globus pallidus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	High field T2-weighted sequences disclosed hypersignal bilateral and symmetrically located exclusively at substantia nigra ( 3 cases ) , exclusively at globus pallidus ( 1case ) and simultaneously at substantia nigra , globus pallidus and nigro-strital interconnections ( 1case ) .
	manualset3
86358	5	398531	13	NULL	NULL	0	NULL	1case	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	High field T2-weighted sequences disclosed hypersignal bilateral and symmetrically located exclusively at substantia nigra ( 3 cases ) , exclusively at globus pallidus ( 1case ) and simultaneously at substantia nigra , globus pallidus and nigro-strital interconnections ( 1case ) .
	manualset3
86359	6	398531	13	NULL	NULL	0	NULL	substantia nigra	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	High field T2-weighted sequences disclosed hypersignal bilateral and symmetrically located exclusively at substantia nigra ( 3 cases ) , exclusively at globus pallidus ( 1case ) and simultaneously at substantia nigra , globus pallidus and nigro-strital interconnections ( 1case ) .
	manualset3
86360	7	398531	13	NULL	NULL	0	NULL	globus pallidus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	High field T2-weighted sequences disclosed hypersignal bilateral and symmetrically located exclusively at substantia nigra ( 3 cases ) , exclusively at globus pallidus ( 1case ) and simultaneously at substantia nigra , globus pallidus and nigro-strital interconnections ( 1case ) .
	manualset3
86361	8	398531	13	NULL	NULL	0	NULL	nigro-strital interconnections	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	High field T2-weighted sequences disclosed hypersignal bilateral and symmetrically located exclusively at substantia nigra ( 3 cases ) , exclusively at globus pallidus ( 1case ) and simultaneously at substantia nigra , globus pallidus and nigro-strital interconnections ( 1case ) .
	manualset3
86362	9	398531	13	NULL	NULL	0	NULL	1case	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	High field T2-weighted sequences disclosed hypersignal bilateral and symmetrically located exclusively at substantia nigra ( 3 cases ) , exclusively at globus pallidus ( 1case ) and simultaneously at substantia nigra , globus pallidus and nigro-strital interconnections ( 1case ) .
	manualset3
86363	1	398532	13	NULL	NULL	0	NULL	High huAbeta/heme ratio	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	High huAbeta/heme ratio increases the peroxidase activity .
	manualset3
86364	2	398532	13	NULL	NULL	0	NULL	peroxidase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	High huAbeta/heme ratio increases the peroxidase activity .
	manualset3
86365	1	398533	13	NULL	NULL	0	NULL	High intake of palatable food	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	High intake of palatable food predicts binge-eating independent of susceptibility to obesity : an animal model of lean vs obese binge-eating and obesity with and without binge-eating .
	manualset3
86366	2	398533	13	NULL	NULL	0	NULL	binge-eating 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	High intake of palatable food predicts binge-eating independent of susceptibility to obesity : an animal model of lean vs obese binge-eating and obesity with and without binge-eating .
	manualset3
86367	3	398533	13	NULL	NULL	0	NULL	susceptibility to obesity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	High intake of palatable food predicts binge-eating independent of susceptibility to obesity : an animal model of lean vs obese binge-eating and obesity with and without binge-eating .
	manualset3
86368	4	398533	13	NULL	NULL	0	NULL	animal model	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	High intake of palatable food predicts binge-eating independent of susceptibility to obesity : an animal model of lean vs obese binge-eating and obesity with and without binge-eating .
	manualset3
86369	5	398533	13	NULL	NULL	0	NULL	lean vs obese binge-eating	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	High intake of palatable food predicts binge-eating independent of susceptibility to obesity : an animal model of lean vs obese binge-eating and obesity with and without binge-eating .
	manualset3
86370	6	398533	13	NULL	NULL	0	NULL	obesity with and without binge-eating	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	High intake of palatable food predicts binge-eating independent of susceptibility to obesity : an animal model of lean vs obese binge-eating and obesity with and without binge-eating .
	manualset3
86371	1	398534	13	NULL	NULL	NULL	NULL	HU protein 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	High levels of HU protein ( 136 molecules/oriC ) restrain the free superhelicity .
	manualset3
86372	2	398534	13	NULL	NULL	0	NULL	136 molecules/oriC 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	High levels of HU protein ( 136 molecules/oriC ) restrain the free superhelicity .
	manualset3
86373	3	398534	13	NULL	NULL	0	NULL	 superhelicity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	High levels of HU protein ( 136 molecules/oriC ) restrain the free superhelicity .
	manualset3
86374	1	398535	13	NULL	NULL	0	NULL	High levels of soluble endothelial protein C receptor ( EPCR )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	High levels of soluble endothelial protein C receptor ( EPCR ) induce coagulation dysfunction by inhibiting protein C activation , and activated protein C ( APC ) activity .
	manualset3
86375	2	398535	13	NULL	NULL	0	NULL	coagulation dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	High levels of soluble endothelial protein C receptor ( EPCR ) induce coagulation dysfunction by inhibiting protein C activation , and activated protein C ( APC ) activity .
	manualset3
86376	3	398535	13	NULL	NULL	0	NULL	protein C activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	High levels of soluble endothelial protein C receptor ( EPCR ) induce coagulation dysfunction by inhibiting protein C activation , and activated protein C ( APC ) activity .
	manualset3
86377	4	398535	13	NULL	NULL	0	NULL	activated protein C ( APC ) activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	High levels of soluble endothelial protein C receptor ( EPCR ) induce coagulation dysfunction by inhibiting protein C activation , and activated protein C ( APC ) activity .
	manualset3
86378	1	398536	13	NULL	NULL	0	NULL	High levels of sunshine exposure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	High levels of sunshine exposure reduced risk of rectal cancer among those diagnosed when & lt ; 60 years of age ( OR = 0.62 , 95 % CI = 0.42-0 .93 ) .
	manualset3
86379	2	398536	13	NULL	NULL	0	NULL	risk of rectal cancer	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	High levels of sunshine exposure reduced risk of rectal cancer among those diagnosed when & lt ; 60 years of age ( OR = 0.62 , 95 % CI = 0.42-0 .93 ) .
	manualset3
86380	3	398536	13	NULL	NULL	0	NULL	60 years of age 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	High levels of sunshine exposure reduced risk of rectal cancer among those diagnosed when & lt ; 60 years of age ( OR = 0.62 , 95 % CI = 0.42-0 .93 ) .
	manualset3
86381	4	398536	13	NULL	NULL	0	NULL	( OR = 0.62 , 95 % CI = 0.42-0 .93 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	High levels of sunshine exposure reduced risk of rectal cancer among those diagnosed when & lt ; 60 years of age ( OR = 0.62 , 95 % CI = 0.42-0 .93 ) .
	manualset3
86382	1	398537	13	NULL	NULL	NULL	NULL	High neuroleptic dosage	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	High neuroleptic dosage was found to be associated with increased reaction time , reduced span of apprehension , low basal skin conductance level , and reduced skin conductance reactivity .
	manualset3
86383	2	398537	13	NULL	NULL	0	NULL	increased reaction time	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	High neuroleptic dosage was found to be associated with increased reaction time , reduced span of apprehension , low basal skin conductance level , and reduced skin conductance reactivity .
	manualset3
86384	3	398537	13	NULL	NULL	0	NULL	reduced span of apprehension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	High neuroleptic dosage was found to be associated with increased reaction time , reduced span of apprehension , low basal skin conductance level , and reduced skin conductance reactivity .
	manualset3
86385	4	398537	13	NULL	NULL	0	NULL	low basal skin conductance level	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	High neuroleptic dosage was found to be associated with increased reaction time , reduced span of apprehension , low basal skin conductance level , and reduced skin conductance reactivity .
	manualset3
86386	5	398537	13	NULL	NULL	0	NULL	reduced skin conductance reactivity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	High neuroleptic dosage was found to be associated with increased reaction time , reduced span of apprehension , low basal skin conductance level , and reduced skin conductance reactivity .
	manualset3
86387	1	398538	13	NULL	NULL	0	NULL	High neutrophilia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	High neutrophilia ( 150 , 000-240 , 000 white blood cell count ) observed in two patients with non-small cell lung cancer led us to run the present trial .
	manualset3
86388	2	398538	13	NULL	NULL	0	NULL	150 , 000-240 , 000 white blood cell count	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	High neutrophilia ( 150 , 000-240 , 000 white blood cell count ) observed in two patients with non-small cell lung cancer led us to run the present trial .
	manualset3
86389	3	398538	13	NULL	NULL	0	NULL	two patients	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	High neutrophilia ( 150 , 000-240 , 000 white blood cell count ) observed in two patients with non-small cell lung cancer led us to run the present trial .
	manualset3
86390	4	398538	13	NULL	NULL	0	NULL	non-small cell lung cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	High neutrophilia ( 150 , 000-240 , 000 white blood cell count ) observed in two patients with non-small cell lung cancer led us to run the present trial .
	manualset3
86391	1	398539	13	NULL	NULL	0	NULL	High prevalence of human rhinovirus C infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	High prevalence of human rhinovirus C infection in Thai children with acute lower respiratory tract disease .
	manualset3
86392	2	398539	13	NULL	NULL	0	NULL	Thai children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	High prevalence of human rhinovirus C infection in Thai children with acute lower respiratory tract disease .
	manualset3
86393	3	398539	13	NULL	NULL	0	NULL	acute lower respiratory tract disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	High prevalence of human rhinovirus C infection in Thai children with acute lower respiratory tract disease .
	manualset3
86394	1	398540	13	NULL	NULL	0	NULL	proline	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	High proline concentration in the youngest uppermost leaves contributed to their protection from drought , which was associated with low degree of senescence .
	manualset3
86395	2	398540	13	NULL	NULL	0	NULL	youngest uppermost leaves	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	High proline concentration in the youngest uppermost leaves contributed to their protection from drought , which was associated with low degree of senescence .
	manualset3
86396	3	398540	13	NULL	NULL	NULL	NULL	drought	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	High proline concentration in the youngest uppermost leaves contributed to their protection from drought , which was associated with low degree of senescence .
	manualset3
86397	4	398540	13	NULL	NULL	0	NULL	low degree of senescence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	High proline concentration in the youngest uppermost leaves contributed to their protection from drought , which was associated with low degree of senescence .
	manualset3
86403	1	398541	13	NULL	NULL	NULL	NULL	High resolution images of the computed full wave field 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	High resolution images of the computed full wave field provide insights into the spiked and rounded features seen in sonic booms that have propagated through turbulence .
	manualset3
86404	2	398541	13	NULL	NULL	0	NULL	sonic booms 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	High resolution images of the computed full wave field provide insights into the spiked and rounded features seen in sonic booms that have propagated through turbulence .
	manualset3
86405	3	398541	13	NULL	NULL	0	NULL	turbulence 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	High resolution images of the computed full wave field provide insights into the spiked and rounded features seen in sonic booms that have propagated through turbulence .
	manualset3
86406	1	398542	13	NULL	NULL	0	NULL	bacterioplankton communities	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	High similarities of the bacterioplankton communities across several hundred kilometers were observed in the surface water using RNA - and DNA-based fingerprints .
	manualset3
86407	2	398542	13	NULL	NULL	0	NULL	several hundred kilometers	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	High similarities of the bacterioplankton communities across several hundred kilometers were observed in the surface water using RNA - and DNA-based fingerprints .
	manualset3
86408	3	398542	13	NULL	NULL	0	NULL	surface water	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	High similarities of the bacterioplankton communities across several hundred kilometers were observed in the surface water using RNA - and DNA-based fingerprints .
	manualset3
86409	4	398542	13	NULL	NULL	0	NULL	RNA -based fingerprints	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	High similarities of the bacterioplankton communities across several hundred kilometers were observed in the surface water using RNA - and DNA-based fingerprints .
	manualset3
86410	5	398542	13	NULL	NULL	0	NULL	DNA-based fingerprints 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	High similarities of the bacterioplankton communities across several hundred kilometers were observed in the surface water using RNA - and DNA-based fingerprints .
	manualset3
86411	1	398543	13	NULL	NULL	0	NULL	similarities	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	High similarities were observed in helminth populations of two groups of states : 1 ) Alabama , Mississippi , Arkansas , Virginia , and Tennessee ; and 2 ) Tennessee , Kentucky , and Illinois .
	manualset3
86412	2	398543	13	NULL	NULL	0	NULL	helminth populations 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	High similarities were observed in helminth populations of two groups of states : 1 ) Alabama , Mississippi , Arkansas , Virginia , and Tennessee ; and 2 ) Tennessee , Kentucky , and Illinois .
	manualset3
86413	3	398543	13	NULL	NULL	0	NULL	 two groups of states	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	High similarities were observed in helminth populations of two groups of states : 1 ) Alabama , Mississippi , Arkansas , Virginia , and Tennessee ; and 2 ) Tennessee , Kentucky , and Illinois .
	manualset3
86414	4	398543	13	NULL	NULL	NULL	NULL	Alabama , Mississippi , Arkansas , Virginia , and Tennessee	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	High similarities were observed in helminth populations of two groups of states : 1 ) Alabama , Mississippi , Arkansas , Virginia , and Tennessee ; and 2 ) Tennessee , Kentucky , and Illinois .
	manualset3
86415	5	398543	13	NULL	NULL	0	NULL	Tennessee , Kentucky , and Illinois 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	High similarities were observed in helminth populations of two groups of states : 1 ) Alabama , Mississippi , Arkansas , Virginia , and Tennessee ; and 2 ) Tennessee , Kentucky , and Illinois .
	manualset3
86416	1	398544	13	NULL	NULL	0	NULL	High street oral surgeons 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	High street oral surgeons -- if the USA catches a cold will the UK get pneumonia ?
	manualset3
86417	2	398544	13	NULL	NULL	0	NULL	USA	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	High street oral surgeons -- if the USA catches a cold will the UK get pneumonia ?
	manualset3
86418	3	398544	13	NULL	NULL	0	NULL	cold 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	High street oral surgeons -- if the USA catches a cold will the UK get pneumonia ?
	manualset3
86419	4	398544	13	NULL	NULL	0	NULL	UK	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	High street oral surgeons -- if the USA catches a cold will the UK get pneumonia ?
	manualset3
86420	5	398544	13	NULL	NULL	0	NULL	pneumonia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	High street oral surgeons -- if the USA catches a cold will the UK get pneumonia ?
	manualset3
86421	1	398545	13	NULL	NULL	0	NULL	university graduates	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	High unemployment of university graduates , a growing factor in developing and developed nations , is pointed to as a major stress during a university education in the late 1970s .
	manualset3
86422	2	398545	13	NULL	NULL	0	NULL	 developing nations 	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	High unemployment of university graduates , a growing factor in developing and developed nations , is pointed to as a major stress during a university education in the late 1970s .
	manualset3
86423	3	398545	13	NULL	NULL	0	NULL	developed nations 	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	High unemployment of university graduates , a growing factor in developing and developed nations , is pointed to as a major stress during a university education in the late 1970s .
	manualset3
86424	4	398545	13	NULL	NULL	0	NULL	major stress	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	High unemployment of university graduates , a growing factor in developing and developed nations , is pointed to as a major stress during a university education in the late 1970s .
	manualset3
86425	5	398545	13	NULL	NULL	0	NULL	university education	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	High unemployment of university graduates , a growing factor in developing and developed nations , is pointed to as a major stress during a university education in the late 1970s .
	manualset3
86426	6	398545	13	NULL	NULL	0	NULL	late 1970s	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	High unemployment of university graduates , a growing factor in developing and developed nations , is pointed to as a major stress during a university education in the late 1970s .
	manualset3
86427	1	398546	13	NULL	NULL	0	NULL	Higher DPP4 gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher DPP4 gene expression in VAT and its relationship with the plasma lipid profile may be explained by actually unknown DPP4 biological effect or , to another extent , may also be a marker of VAT inflammation known to be associated with metabolic disturbances .
	manualset3
86428	2	398546	13	NULL	NULL	0	NULL	VAT	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher DPP4 gene expression in VAT and its relationship with the plasma lipid profile may be explained by actually unknown DPP4 biological effect or , to another extent , may also be a marker of VAT inflammation known to be associated with metabolic disturbances .
	manualset3
86429	3	398546	13	NULL	NULL	NULL	NULL	plasma lipid profile 	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Higher DPP4 gene expression in VAT and its relationship with the plasma lipid profile may be explained by actually unknown DPP4 biological effect or , to another extent , may also be a marker of VAT inflammation known to be associated with metabolic disturbances .
	manualset3
86430	4	398546	13	NULL	NULL	0	NULL	DPP4 biological effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher DPP4 gene expression in VAT and its relationship with the plasma lipid profile may be explained by actually unknown DPP4 biological effect or , to another extent , may also be a marker of VAT inflammation known to be associated with metabolic disturbances .
	manualset3
86431	5	398546	13	NULL	NULL	0	NULL	VAT inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher DPP4 gene expression in VAT and its relationship with the plasma lipid profile may be explained by actually unknown DPP4 biological effect or , to another extent , may also be a marker of VAT inflammation known to be associated with metabolic disturbances .
	manualset3
86432	6	398546	13	NULL	NULL	0	NULL	metabolic disturbances	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher DPP4 gene expression in VAT and its relationship with the plasma lipid profile may be explained by actually unknown DPP4 biological effect or , to another extent , may also be a marker of VAT inflammation known to be associated with metabolic disturbances .
	manualset3
86433	7	398546	13	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher DPP4 gene expression in VAT and its relationship with the plasma lipid profile may be explained by actually unknown DPP4 biological effect or , to another extent , may also be a marker of VAT inflammation known to be associated with metabolic disturbances .
	manualset3
86434	1	398547	13	NULL	NULL	0	NULL	Ki-67 expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher Ki-67 expression in immunostaining and RT-PCR was more often seen in grade 3 tumors ( p & lt ; 0.001 and p = 0.026 , respectively ) .
	manualset3
86435	2	398547	13	NULL	NULL	0	NULL	immunostaining	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher Ki-67 expression in immunostaining and RT-PCR was more often seen in grade 3 tumors ( p & lt ; 0.001 and p = 0.026 , respectively ) .
	manualset3
86436	3	398547	13	NULL	NULL	0	NULL	RT-PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher Ki-67 expression in immunostaining and RT-PCR was more often seen in grade 3 tumors ( p & lt ; 0.001 and p = 0.026 , respectively ) .
	manualset3
86437	4	398547	13	NULL	NULL	0	NULL	grade 3 tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher Ki-67 expression in immunostaining and RT-PCR was more often seen in grade 3 tumors ( p & lt ; 0.001 and p = 0.026 , respectively ) .
	manualset3
86438	5	398547	13	NULL	NULL	0	NULL	 p & lt ; 0.001 and p = 0.026 , respectively	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher Ki-67 expression in immunostaining and RT-PCR was more often seen in grade 3 tumors ( p & lt ; 0.001 and p = 0.026 , respectively ) .
	manualset3
86439	1	398548	13	NULL	NULL	0	NULL	Higher fees	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher fees have been implemented for rural transports and air ambulance services .
	manualset3
86440	2	398548	13	NULL	NULL	0	NULL	rural transports 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher fees have been implemented for rural transports and air ambulance services .
	manualset3
86441	3	398548	13	NULL	NULL	0	NULL	air ambulance services	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher fees have been implemented for rural transports and air ambulance services .
	manualset3
86442	1	398549	13	NULL	NULL	NULL	NULL	Higher kidney weights	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Higher kidney weights , correlating to renal tubule hypertrophy in the 0.6 mg/kg group , were observed for parental males and females in the 0.125 and 0.6 mg / ( kgday ) groups .
	manualset3
86443	2	398549	13	NULL	NULL	0	NULL	renal tubule hypertrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher kidney weights , correlating to renal tubule hypertrophy in the 0.6 mg/kg group , were observed for parental males and females in the 0.125 and 0.6 mg / ( kgday ) groups .
	manualset3
86444	3	398549	13	NULL	NULL	NULL	NULL	0.6 mg/kg group	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Higher kidney weights , correlating to renal tubule hypertrophy in the 0.6 mg/kg group , were observed for parental males and females in the 0.125 and 0.6 mg / ( kgday ) groups .
	manualset3
86445	4	398549	13	NULL	NULL	0	NULL	parental males	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher kidney weights , correlating to renal tubule hypertrophy in the 0.6 mg/kg group , were observed for parental males and females in the 0.125 and 0.6 mg / ( kgday ) groups .
	manualset3
86446	5	398549	13	NULL	NULL	NULL	NULL	parental females	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Higher kidney weights , correlating to renal tubule hypertrophy in the 0.6 mg/kg group , were observed for parental males and females in the 0.125 and 0.6 mg / ( kgday ) groups .
	manualset3
86447	6	398549	13	NULL	NULL	0	NULL	0.125 mg / ( kgday ) group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher kidney weights , correlating to renal tubule hypertrophy in the 0.6 mg/kg group , were observed for parental males and females in the 0.125 and 0.6 mg / ( kgday ) groups .
	manualset3
86448	7	398549	13	NULL	NULL	0	NULL	0.6 mg / ( kgday ) group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher kidney weights , correlating to renal tubule hypertrophy in the 0.6 mg/kg group , were observed for parental males and females in the 0.125 and 0.6 mg / ( kgday ) groups .
	manualset3
86449	1	398550	13	NULL	NULL	0	NULL	Higher neuroticism scores	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher neuroticism scores also attenuated the decrease in negative affect across time .
	manualset3
86450	2	398550	13	NULL	NULL	0	NULL	 decrease in negative affect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher neuroticism scores also attenuated the decrease in negative affect across time .
	manualset3
86451	3	398550	13	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher neuroticism scores also attenuated the decrease in negative affect across time .
	manualset3
86452	1	398551	13	NULL	NULL	0	NULL	Higher rates of refractory infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher rates of refractory infection , serious morbidity , and attributable death occurred in the VREF cohort and were partially mediated by the lack of effective antimicrobial therapy .
	manualset3
86453	2	398551	13	NULL	NULL	0	NULL	serious morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher rates of refractory infection , serious morbidity , and attributable death occurred in the VREF cohort and were partially mediated by the lack of effective antimicrobial therapy .
	manualset3
86454	3	398551	13	NULL	NULL	0	NULL	attributable death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher rates of refractory infection , serious morbidity , and attributable death occurred in the VREF cohort and were partially mediated by the lack of effective antimicrobial therapy .
	manualset3
86462	4	398551	13	NULL	NULL	0	NULL	VREF cohort	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher rates of refractory infection , serious morbidity , and attributable death occurred in the VREF cohort and were partially mediated by the lack of effective antimicrobial therapy .
	manualset3
86463	5	398551	13	NULL	NULL	0	NULL	antimicrobial therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher rates of refractory infection , serious morbidity , and attributable death occurred in the VREF cohort and were partially mediated by the lack of effective antimicrobial therapy .
	manualset3
86464	1	398552	13	NULL	NULL	NULL	NULL	urban setting	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Higher rates were found in urban than rural setting and , to a lesser degree , for women than men .
	manualset3
86465	2	398552	13	NULL	NULL	0	NULL	rural setting	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher rates were found in urban than rural setting and , to a lesser degree , for women than men .
	manualset3
86466	3	398552	13	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher rates were found in urban than rural setting and , to a lesser degree , for women than men .
	manualset3
86467	4	398552	13	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher rates were found in urban than rural setting and , to a lesser degree , for women than men .
	manualset3
86468	1	398553	13	NULL	NULL	0	NULL	Higher susceptibility to peroxidation in heart 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher susceptibility to peroxidation in heart , thymus and pancreas was also found in the sucrose-fed group v. the starch-fed group .
	manualset3
86469	2	398553	13	NULL	NULL	0	NULL	Higher susceptibility to peroxidation in thymus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher susceptibility to peroxidation in heart , thymus and pancreas was also found in the sucrose-fed group v. the starch-fed group .
	manualset3
86470	3	398553	13	NULL	NULL	0	NULL	Higher susceptibility to peroxidation in pancreas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher susceptibility to peroxidation in heart , thymus and pancreas was also found in the sucrose-fed group v. the starch-fed group .
	manualset3
86471	4	398553	13	NULL	NULL	0	NULL	sucrose-fed group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher susceptibility to peroxidation in heart , thymus and pancreas was also found in the sucrose-fed group v. the starch-fed group .
	manualset3
86472	5	398553	13	NULL	NULL	0	NULL	starch-fed group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher susceptibility to peroxidation in heart , thymus and pancreas was also found in the sucrose-fed group v. the starch-fed group .
	manualset3
86473	1	398554	13	NULL	NULL	0	NULL	Higher values of seminiferous tubule diameters	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher values of seminiferous tubule diameters and all types of spermatogenic cells including mature-phase spermatozoa were found during the breeding season .
	manualset3
86474	2	398554	13	NULL	NULL	0	NULL	all types of spermatogenic cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher values of seminiferous tubule diameters and all types of spermatogenic cells including mature-phase spermatozoa were found during the breeding season .
	manualset3
86475	3	398554	13	NULL	NULL	0	NULL	mature-phase spermatozoa	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher values of seminiferous tubule diameters and all types of spermatogenic cells including mature-phase spermatozoa were found during the breeding season .
	manualset3
86476	4	398554	13	NULL	NULL	0	NULL	breeding season	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Higher values of seminiferous tubule diameters and all types of spermatogenic cells including mature-phase spermatozoa were found during the breeding season .
	manualset3
86477	1	398555	13	NULL	NULL	0	NULL	Highest 3H-naloxone binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Highest 3H-naloxone binding occurs in the inferior olive in fetuses at midgestation , compared to the interpeduncular nucleus in infants .
	manualset3
86478	2	398555	13	NULL	NULL	0	NULL	inferior olive	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Highest 3H-naloxone binding occurs in the inferior olive in fetuses at midgestation , compared to the interpeduncular nucleus in infants .
	manualset3
86479	3	398555	13	NULL	NULL	0	NULL	fetuses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Highest 3H-naloxone binding occurs in the inferior olive in fetuses at midgestation , compared to the interpeduncular nucleus in infants .
	manualset3
86480	4	398555	13	NULL	NULL	0	NULL	midgestation	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Highest 3H-naloxone binding occurs in the inferior olive in fetuses at midgestation , compared to the interpeduncular nucleus in infants .
	manualset3
86481	5	398555	13	NULL	NULL	0	NULL	interpeduncular nucleus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Highest 3H-naloxone binding occurs in the inferior olive in fetuses at midgestation , compared to the interpeduncular nucleus in infants .
	manualset3
86482	6	398555	13	NULL	NULL	0	NULL	infants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Highest 3H-naloxone binding occurs in the inferior olive in fetuses at midgestation , compared to the interpeduncular nucleus in infants .
	manualset3
86483	1	398556	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Highest levels were seen in patients with active systemic JRA ( mean value 2419 U/ml ) while patients with pauciarticular JRA and B27 + JRA had the lowest sIL-2R levels ( 1167 and 1045 U/ml , respectively ) .
	manualset3
86490	2	398556	13	NULL	NULL	0	NULL	active systemic JRA	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Highest levels were seen in patients with active systemic JRA ( mean value 2419 U/ml ) while patients with pauciarticular JRA and B27 + JRA had the lowest sIL-2R levels ( 1167 and 1045 U/ml , respectively ) .
	manualset3
86491	3	398556	13	NULL	NULL	0	NULL	 mean value 2419 U/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Highest levels were seen in patients with active systemic JRA ( mean value 2419 U/ml ) while patients with pauciarticular JRA and B27 + JRA had the lowest sIL-2R levels ( 1167 and 1045 U/ml , respectively ) .
	manualset3
86492	4	398556	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Highest levels were seen in patients with active systemic JRA ( mean value 2419 U/ml ) while patients with pauciarticular JRA and B27 + JRA had the lowest sIL-2R levels ( 1167 and 1045 U/ml , respectively ) .
	manualset3
86494	5	398556	13	NULL	NULL	0	NULL	pauciarticular JRA	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Highest levels were seen in patients with active systemic JRA ( mean value 2419 U/ml ) while patients with pauciarticular JRA and B27 + JRA had the lowest sIL-2R levels ( 1167 and 1045 U/ml , respectively ) .
	manualset3
86495	6	398556	13	NULL	NULL	0	NULL	B27 + JRA	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Highest levels were seen in patients with active systemic JRA ( mean value 2419 U/ml ) while patients with pauciarticular JRA and B27 + JRA had the lowest sIL-2R levels ( 1167 and 1045 U/ml , respectively ) .
	manualset3
86496	7	398556	13	NULL	NULL	0	NULL	lowest sIL-2R levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Highest levels were seen in patients with active systemic JRA ( mean value 2419 U/ml ) while patients with pauciarticular JRA and B27 + JRA had the lowest sIL-2R levels ( 1167 and 1045 U/ml , respectively ) .
	manualset3
86497	8	398556	13	NULL	NULL	0	NULL	1167 U/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Highest levels were seen in patients with active systemic JRA ( mean value 2419 U/ml ) while patients with pauciarticular JRA and B27 + JRA had the lowest sIL-2R levels ( 1167 and 1045 U/ml , respectively ) .
	manualset3
86498	9	398556	13	NULL	NULL	0	NULL	1045 U/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Highest levels were seen in patients with active systemic JRA ( mean value 2419 U/ml ) while patients with pauciarticular JRA and B27 + JRA had the lowest sIL-2R levels ( 1167 and 1045 U/ml , respectively ) .
	manualset3
86499	1	398557	13	NULL	NULL	0	NULL	pyrene mineralization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Highest pyrene mineralization rates and extents ( more than 60 % after 20 days ) were obtained when pyrene was in contact with composted soil from the curing stage .
	manualset3
86500	2	398557	13	NULL	NULL	0	NULL	 more than 60 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Highest pyrene mineralization rates and extents ( more than 60 % after 20 days ) were obtained when pyrene was in contact with composted soil from the curing stage .
	manualset3
86501	3	398557	13	NULL	NULL	NULL	NULL	after 20 days 	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Highest pyrene mineralization rates and extents ( more than 60 % after 20 days ) were obtained when pyrene was in contact with composted soil from the curing stage .
	manualset3
86502	4	398557	13	NULL	NULL	NULL	NULL	pyrene	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Highest pyrene mineralization rates and extents ( more than 60 % after 20 days ) were obtained when pyrene was in contact with composted soil from the curing stage .
	manualset3
86503	5	398557	13	NULL	NULL	0	NULL	composted soil	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Highest pyrene mineralization rates and extents ( more than 60 % after 20 days ) were obtained when pyrene was in contact with composted soil from the curing stage .
	manualset3
86504	6	398557	13	NULL	NULL	0	NULL	curing stage	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Highest pyrene mineralization rates and extents ( more than 60 % after 20 days ) were obtained when pyrene was in contact with composted soil from the curing stage .
	manualset3
86505	1	398558	13	NULL	NULL	0	NULL	printed fuel cell	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Highest stability was obtained for a printed fuel cell using osmium complexes as mediators of glucose oxidation by aldose dehydrogenase , and oxygen reduction by T. hirsuta laccase , maintaining cell voltage above 200mV for 137h at pH 5 .
	manualset3
86506	2	398558	13	NULL	NULL	0	NULL	osmium complexes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Highest stability was obtained for a printed fuel cell using osmium complexes as mediators of glucose oxidation by aldose dehydrogenase , and oxygen reduction by T. hirsuta laccase , maintaining cell voltage above 200mV for 137h at pH 5 .
	manualset3
86507	3	398558	13	NULL	NULL	0	NULL	mediators	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Highest stability was obtained for a printed fuel cell using osmium complexes as mediators of glucose oxidation by aldose dehydrogenase , and oxygen reduction by T. hirsuta laccase , maintaining cell voltage above 200mV for 137h at pH 5 .
	manualset3
86508	4	398558	13	NULL	NULL	0	NULL	glucose oxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Highest stability was obtained for a printed fuel cell using osmium complexes as mediators of glucose oxidation by aldose dehydrogenase , and oxygen reduction by T. hirsuta laccase , maintaining cell voltage above 200mV for 137h at pH 5 .
	manualset3
86509	5	398558	13	NULL	NULL	0	NULL	aldose dehydrogenase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Highest stability was obtained for a printed fuel cell using osmium complexes as mediators of glucose oxidation by aldose dehydrogenase , and oxygen reduction by T. hirsuta laccase , maintaining cell voltage above 200mV for 137h at pH 5 .
	manualset3
86510	6	398558	13	NULL	NULL	0	NULL	oxygen reduction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Highest stability was obtained for a printed fuel cell using osmium complexes as mediators of glucose oxidation by aldose dehydrogenase , and oxygen reduction by T. hirsuta laccase , maintaining cell voltage above 200mV for 137h at pH 5 .
	manualset3
86511	7	398558	13	NULL	NULL	0	NULL	T. hirsuta laccase	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Highest stability was obtained for a printed fuel cell using osmium complexes as mediators of glucose oxidation by aldose dehydrogenase , and oxygen reduction by T. hirsuta laccase , maintaining cell voltage above 200mV for 137h at pH 5 .
	manualset3
86512	8	398558	13	NULL	NULL	0	NULL	cell 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Highest stability was obtained for a printed fuel cell using osmium complexes as mediators of glucose oxidation by aldose dehydrogenase , and oxygen reduction by T. hirsuta laccase , maintaining cell voltage above 200mV for 137h at pH 5 .
	manualset3
86513	9	398558	13	NULL	NULL	0	NULL	voltage above 200mV	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Highest stability was obtained for a printed fuel cell using osmium complexes as mediators of glucose oxidation by aldose dehydrogenase , and oxygen reduction by T. hirsuta laccase , maintaining cell voltage above 200mV for 137h at pH 5 .
	manualset3
86514	10	398558	13	NULL	NULL	0	NULL	137h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Highest stability was obtained for a printed fuel cell using osmium complexes as mediators of glucose oxidation by aldose dehydrogenase , and oxygen reduction by T. hirsuta laccase , maintaining cell voltage above 200mV for 137h at pH 5 .
	manualset3
86515	11	398558	13	NULL	NULL	0	NULL	pH 5	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Highest stability was obtained for a printed fuel cell using osmium complexes as mediators of glucose oxidation by aldose dehydrogenase , and oxygen reduction by T. hirsuta laccase , maintaining cell voltage above 200mV for 137h at pH 5 .
	manualset3
86516	1	398559	13	NULL	NULL	0	NULL	modified vaccinia virus Ankara ( MVA )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly attenuated modified vaccinia virus Ankara ( MVA ) as an effective recombinant vector : a murine tumor model .
	manualset3
86517	2	398559	13	NULL	NULL	NULL	NULL	recombinant vector	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Highly attenuated modified vaccinia virus Ankara ( MVA ) as an effective recombinant vector : a murine tumor model .
	manualset3
86518	3	398559	13	NULL	NULL	0	NULL	 murine tumor model 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly attenuated modified vaccinia virus Ankara ( MVA ) as an effective recombinant vector : a murine tumor model .
	manualset3
86519	1	398560	13	NULL	NULL	NULL	NULL	Highly conserved regions	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Highly conserved regions were observed among the deduced amino acid sequences of AT1 , AT2 , chicken erythroblast and rabbit and human skeletal muscle ADP-ribosyltransferases , and rodent T-cell surface antigen RT6 .
	manualset3
86520	2	398560	13	NULL	NULL	NULL	NULL	amino acid sequences of AT1	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Highly conserved regions were observed among the deduced amino acid sequences of AT1 , AT2 , chicken erythroblast and rabbit and human skeletal muscle ADP-ribosyltransferases , and rodent T-cell surface antigen RT6 .
	manualset3
86521	3	398560	13	NULL	NULL	NULL	NULL	AT2	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Highly conserved regions were observed among the deduced amino acid sequences of AT1 , AT2 , chicken erythroblast and rabbit and human skeletal muscle ADP-ribosyltransferases , and rodent T-cell surface antigen RT6 .
	manualset3
86522	4	398560	13	NULL	NULL	NULL	NULL	chicken erythroblast ADP-ribosyltransferase	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Highly conserved regions were observed among the deduced amino acid sequences of AT1 , AT2 , chicken erythroblast and rabbit and human skeletal muscle ADP-ribosyltransferases , and rodent T-cell surface antigen RT6 .
	manualset3
86523	5	398560	13	NULL	NULL	0	NULL	rabbit ADP-ribosyltransferase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly conserved regions were observed among the deduced amino acid sequences of AT1 , AT2 , chicken erythroblast and rabbit and human skeletal muscle ADP-ribosyltransferases , and rodent T-cell surface antigen RT6 .
	manualset3
86524	6	398560	13	NULL	NULL	0	NULL	human skeletal muscle ADP-ribosyltransferase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly conserved regions were observed among the deduced amino acid sequences of AT1 , AT2 , chicken erythroblast and rabbit and human skeletal muscle ADP-ribosyltransferases , and rodent T-cell surface antigen RT6 .
	manualset3
86525	7	398560	13	NULL	NULL	0	NULL	rodent T-cell surface antigen RT6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly conserved regions were observed among the deduced amino acid sequences of AT1 , AT2 , chicken erythroblast and rabbit and human skeletal muscle ADP-ribosyltransferases , and rodent T-cell surface antigen RT6 .
	manualset3
86526	1	398561	13	NULL	NULL	0	NULL	Highly crystalline nanostructured multilayered assemblies	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly crystalline nanostructured multilayered assemblies were formed , which revealed a very rich polymorphism of micro - and macro-structures depending on the chemical structure of the bile acid and the properties of the cosolvent ( EtOH or DMSO ) used .
	manualset3
86527	2	398561	13	NULL	NULL	NULL	NULL	polymorphism	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Highly crystalline nanostructured multilayered assemblies were formed , which revealed a very rich polymorphism of micro - and macro-structures depending on the chemical structure of the bile acid and the properties of the cosolvent ( EtOH or DMSO ) used .
	manualset3
86528	3	398561	13	NULL	NULL	NULL	NULL	micro -structures	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Highly crystalline nanostructured multilayered assemblies were formed , which revealed a very rich polymorphism of micro - and macro-structures depending on the chemical structure of the bile acid and the properties of the cosolvent ( EtOH or DMSO ) used .
	manualset3
86529	4	398561	13	NULL	NULL	NULL	NULL	macro-structures	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Highly crystalline nanostructured multilayered assemblies were formed , which revealed a very rich polymorphism of micro - and macro-structures depending on the chemical structure of the bile acid and the properties of the cosolvent ( EtOH or DMSO ) used .
	manualset3
86530	5	398561	13	NULL	NULL	0	NULL	chemical structure of the bile acid	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly crystalline nanostructured multilayered assemblies were formed , which revealed a very rich polymorphism of micro - and macro-structures depending on the chemical structure of the bile acid and the properties of the cosolvent ( EtOH or DMSO ) used .
	manualset3
86531	6	398561	13	NULL	NULL	0	NULL	cosolvent ( EtOH or DMSO )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly crystalline nanostructured multilayered assemblies were formed , which revealed a very rich polymorphism of micro - and macro-structures depending on the chemical structure of the bile acid and the properties of the cosolvent ( EtOH or DMSO ) used .
	manualset3
86532	1	398562	13	NULL	NULL	0	NULL	enantioselective hydrogenation of enol ester phosphonates	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly enantioselective hydrogenation of enol ester phosphonates catalyzed by rhodium phosphine-phosphite complexes .
	manualset3
86533	2	398562	13	NULL	NULL	0	NULL	rhodium phosphine-phosphite complexes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly enantioselective hydrogenation of enol ester phosphonates catalyzed by rhodium phosphine-phosphite complexes .
	manualset3
86534	1	398563	13	NULL	NULL	NULL	NULL	lipidated C14 HSA	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Highly lipidated C14 HSA ( C14 , fatty acid side-chains with 14 carbon atoms ) was not itself mitogenic : unlike HSA it localized heavily to the red pulp as well as to cells of dendritic form in the splenic white pulp .
	manualset3
86535	2	398563	13	NULL	NULL	0	NULL	C14 , fatty acid side-chains with 14 carbon atoms 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly lipidated C14 HSA ( C14 , fatty acid side-chains with 14 carbon atoms ) was not itself mitogenic : unlike HSA it localized heavily to the red pulp as well as to cells of dendritic form in the splenic white pulp .
	manualset3
86536	3	398563	13	NULL	NULL	NULL	NULL	HSA	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Highly lipidated C14 HSA ( C14 , fatty acid side-chains with 14 carbon atoms ) was not itself mitogenic : unlike HSA it localized heavily to the red pulp as well as to cells of dendritic form in the splenic white pulp .
	manualset3
86537	4	398563	13	NULL	NULL	0	NULL	red pulp	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly lipidated C14 HSA ( C14 , fatty acid side-chains with 14 carbon atoms ) was not itself mitogenic : unlike HSA it localized heavily to the red pulp as well as to cells of dendritic form in the splenic white pulp .
	manualset3
86538	5	398563	13	NULL	NULL	0	NULL	cells of dendritic form	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly lipidated C14 HSA ( C14 , fatty acid side-chains with 14 carbon atoms ) was not itself mitogenic : unlike HSA it localized heavily to the red pulp as well as to cells of dendritic form in the splenic white pulp .
	manualset3
86539	6	398563	13	NULL	NULL	0	NULL	splenic white pulp	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly lipidated C14 HSA ( C14 , fatty acid side-chains with 14 carbon atoms ) was not itself mitogenic : unlike HSA it localized heavily to the red pulp as well as to cells of dendritic form in the splenic white pulp .
	manualset3
86540	1	398564	13	NULL	NULL	NULL	NULL	Temperature	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Temperature of adaptation and regeneration in vivo of various molecular species of lecithins of rainbow trout ( Salmo gairdneri R. ) tissues ) .
	manualset3
86541	2	398564	13	NULL	NULL	0	NULL	adaptation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Temperature of adaptation and regeneration in vivo of various molecular species of lecithins of rainbow trout ( Salmo gairdneri R. ) tissues ) .
	manualset3
86542	3	398564	13	NULL	NULL	0	NULL	regeneration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Temperature of adaptation and regeneration in vivo of various molecular species of lecithins of rainbow trout ( Salmo gairdneri R. ) tissues ) .
	manualset3
86543	4	398564	13	NULL	NULL	NULL	NULL	various molecular species of lecithins	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Temperature of adaptation and regeneration in vivo of various molecular species of lecithins of rainbow trout ( Salmo gairdneri R. ) tissues ) .
	manualset3
86544	5	398564	13	NULL	NULL	0	NULL	rainbow trout ( Salmo gairdneri R. ) tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	( Temperature of adaptation and regeneration in vivo of various molecular species of lecithins of rainbow trout ( Salmo gairdneri R. ) tissues ) .
	manualset3
86545	1	398565	13	NULL	NULL	0	NULL	Highly motivated patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly motivated patients had greater improvement on the Stereotypy Linear Analog Scale and Stereotypy Severity Scale scales compared with less motivated patients , but motivation had no impact on the Child Global Assessment Scale .
	manualset3
86546	2	398565	13	NULL	NULL	0	NULL	greater improvement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly motivated patients had greater improvement on the Stereotypy Linear Analog Scale and Stereotypy Severity Scale scales compared with less motivated patients , but motivation had no impact on the Child Global Assessment Scale .
	manualset3
86547	3	398565	13	NULL	NULL	0	NULL	Stereotypy Linear Analog Scale	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly motivated patients had greater improvement on the Stereotypy Linear Analog Scale and Stereotypy Severity Scale scales compared with less motivated patients , but motivation had no impact on the Child Global Assessment Scale .
	manualset3
86548	4	398565	13	NULL	NULL	0	NULL	Stereotypy Severity Scale scales	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly motivated patients had greater improvement on the Stereotypy Linear Analog Scale and Stereotypy Severity Scale scales compared with less motivated patients , but motivation had no impact on the Child Global Assessment Scale .
	manualset3
86549	5	398565	13	NULL	NULL	0	NULL	less motivated patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly motivated patients had greater improvement on the Stereotypy Linear Analog Scale and Stereotypy Severity Scale scales compared with less motivated patients , but motivation had no impact on the Child Global Assessment Scale .
	manualset3
86550	6	398565	13	NULL	NULL	0	NULL	Child Global Assessment Scale	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly motivated patients had greater improvement on the Stereotypy Linear Analog Scale and Stereotypy Severity Scale scales compared with less motivated patients , but motivation had no impact on the Child Global Assessment Scale .
	manualset3
86551	1	398566	13	NULL	NULL	0	NULL	Highly pathogenic infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly pathogenic infections , with long-lived infective stages , tend to produce cyclic behavior in their host populations .
	manualset3
86552	2	398566	13	NULL	NULL	0	NULL	long-lived infective stages	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly pathogenic infections , with long-lived infective stages , tend to produce cyclic behavior in their host populations .
	manualset3
86553	3	398566	13	NULL	NULL	0	NULL	cyclic behavior	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly pathogenic infections , with long-lived infective stages , tend to produce cyclic behavior in their host populations .
	manualset3
86554	4	398566	13	NULL	NULL	0	NULL	host populations	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly pathogenic infections , with long-lived infective stages , tend to produce cyclic behavior in their host populations .
	manualset3
86555	1	398567	13	NULL	NULL	0	NULL	Highly sensitive molecularly imprinted electrochemical sensor	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly sensitive molecularly imprinted electrochemical sensor based on the double amplification by an inorganic Prussian blue catalytic polymer and the enzymatic effect of glucose oxidase .
	manualset3
86556	2	398567	13	NULL	NULL	0	NULL	double amplification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly sensitive molecularly imprinted electrochemical sensor based on the double amplification by an inorganic Prussian blue catalytic polymer and the enzymatic effect of glucose oxidase .
	manualset3
86557	3	398567	13	NULL	NULL	0	NULL	inorganic Prussian blue catalytic polymer	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly sensitive molecularly imprinted electrochemical sensor based on the double amplification by an inorganic Prussian blue catalytic polymer and the enzymatic effect of glucose oxidase .
	manualset3
86558	4	398567	13	NULL	NULL	0	NULL	 enzymatic effect of glucose oxidase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly sensitive molecularly imprinted electrochemical sensor based on the double amplification by an inorganic Prussian blue catalytic polymer and the enzymatic effect of glucose oxidase .
	manualset3
86559	1	398568	13	NULL	NULL	NULL	NULL	Highly successful antimicrobial measures 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Highly successful antimicrobial measures that would reduce the number of diseased sibs independent of the distribution of susceptible sibs could produce a dissociation of the gene-to - `` rheumatic '' relationship and thus explains the declining ascertainment bias .
	manualset3
86560	2	398568	13	NULL	NULL	0	NULL	diseased sibs	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly successful antimicrobial measures that would reduce the number of diseased sibs independent of the distribution of susceptible sibs could produce a dissociation of the gene-to - `` rheumatic '' relationship and thus explains the declining ascertainment bias .
	manualset3
86561	3	398568	13	NULL	NULL	0	NULL	distribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly successful antimicrobial measures that would reduce the number of diseased sibs independent of the distribution of susceptible sibs could produce a dissociation of the gene-to - `` rheumatic '' relationship and thus explains the declining ascertainment bias .
	manualset3
86562	4	398568	13	NULL	NULL	0	NULL	 susceptible sibs	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly successful antimicrobial measures that would reduce the number of diseased sibs independent of the distribution of susceptible sibs could produce a dissociation of the gene-to - `` rheumatic '' relationship and thus explains the declining ascertainment bias .
	manualset3
86563	5	398568	13	NULL	NULL	NULL	NULL	dissociation 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Highly successful antimicrobial measures that would reduce the number of diseased sibs independent of the distribution of susceptible sibs could produce a dissociation of the gene-to - `` rheumatic '' relationship and thus explains the declining ascertainment bias .
	manualset3
86564	6	398568	13	NULL	NULL	NULL	NULL	gene-to - `` rheumatic '' relationship	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Highly successful antimicrobial measures that would reduce the number of diseased sibs independent of the distribution of susceptible sibs could produce a dissociation of the gene-to - `` rheumatic '' relationship and thus explains the declining ascertainment bias .
	manualset3
86565	7	398568	13	NULL	NULL	NULL	NULL	declining ascertainment bias 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Highly successful antimicrobial measures that would reduce the number of diseased sibs independent of the distribution of susceptible sibs could produce a dissociation of the gene-to - `` rheumatic '' relationship and thus explains the declining ascertainment bias .
	manualset3
86566	1	398569	13	NULL	NULL	0	NULL	pi-conjugation extension	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly unusual effects of pi-conjugation extension on the molecular linear and quadratic nonlinear optical properties of ruthenium ( II ) ammine complexes .
	manualset3
86567	2	398569	13	NULL	NULL	0	NULL	ruthenium ( II ) ammine complexes 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly unusual effects of pi-conjugation extension on the molecular linear and quadratic nonlinear optical properties of ruthenium ( II ) ammine complexes .
	manualset3
86568	3	398569	13	NULL	NULL	0	NULL	 molecular linear properties	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly unusual effects of pi-conjugation extension on the molecular linear and quadratic nonlinear optical properties of ruthenium ( II ) ammine complexes .
	manualset3
86569	4	398569	13	NULL	NULL	0	NULL	quadratic nonlinear optical properties 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly unusual effects of pi-conjugation extension on the molecular linear and quadratic nonlinear optical properties of ruthenium ( II ) ammine complexes .
	manualset3
86570	1	398570	13	NULL	NULL	NULL	NULL	Hilbert transform	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hilbert transform is used to combine multiple channel measurements and the adaptive rule based decision process is used to eliminate spurious beats .
	manualset3
86571	2	398570	13	NULL	NULL	NULL	NULL	multiple channel measurements	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hilbert transform is used to combine multiple channel measurements and the adaptive rule based decision process is used to eliminate spurious beats .
	manualset3
86572	3	398570	13	NULL	NULL	NULL	NULL	adaptive rule based decision process	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hilbert transform is used to combine multiple channel measurements and the adaptive rule based decision process is used to eliminate spurious beats .
	manualset3
86574	1	398571	13	NULL	NULL	0	NULL	Hindsight	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hindsight rather than foresight : reality versus the EU draft guideline on pharmaceuticals in the environment .
	manualset3
86575	2	398571	13	NULL	NULL	0	NULL	foresight	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hindsight rather than foresight : reality versus the EU draft guideline on pharmaceuticals in the environment .
	manualset3
86576	3	398571	13	NULL	NULL	0	NULL	EU draft guideline	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Hindsight rather than foresight : reality versus the EU draft guideline on pharmaceuticals in the environment .
	manualset3
86577	4	398571	13	NULL	NULL	0	NULL	pharmaceuticals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hindsight rather than foresight : reality versus the EU draft guideline on pharmaceuticals in the environment .
	manualset3
86578	5	398571	13	NULL	NULL	0	NULL	environment	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Hindsight rather than foresight : reality versus the EU draft guideline on pharmaceuticals in the environment .
	manualset3
86579	1	398572	13	NULL	NULL	0	NULL	 Termination of pregnancy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Termination of pregnancy , a very difficult question ) .
	manualset3
86580	1	398573	13	NULL	NULL	0	NULL	Hippocampal slices	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Hippocampal slices ( 450 microm ) generate epileptiform bursts of an interictal nature when perfused with a zero magnesium medium containing 4-aminopyridine ( 50 microM ) .
	manualset3
86581	2	398573	13	NULL	NULL	0	NULL	450 microm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Hippocampal slices ( 450 microm ) generate epileptiform bursts of an interictal nature when perfused with a zero magnesium medium containing 4-aminopyridine ( 50 microM ) .
	manualset3
86582	3	398573	13	NULL	NULL	0	NULL	generate epileptiform bursts of an interictal nature 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hippocampal slices ( 450 microm ) generate epileptiform bursts of an interictal nature when perfused with a zero magnesium medium containing 4-aminopyridine ( 50 microM ) .
	manualset3
86583	4	398573	13	NULL	NULL	0	NULL	zero magnesium medium	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Hippocampal slices ( 450 microm ) generate epileptiform bursts of an interictal nature when perfused with a zero magnesium medium containing 4-aminopyridine ( 50 microM ) .
	manualset3
86584	5	398573	13	NULL	NULL	NULL	NULL	4-aminopyridine	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hippocampal slices ( 450 microm ) generate epileptiform bursts of an interictal nature when perfused with a zero magnesium medium containing 4-aminopyridine ( 50 microM ) .
	manualset3
86585	6	398573	13	NULL	NULL	NULL	NULL	50 microM	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hippocampal slices ( 450 microm ) generate epileptiform bursts of an interictal nature when perfused with a zero magnesium medium containing 4-aminopyridine ( 50 microM ) .
	manualset3
86586	1	398574	13	NULL	NULL	0	NULL	 generalised fair innings approach 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	His ` generalised fair innings approach ' on the one hand , and the severity approach on the other , are two ways of incorporating concerns for fairness in economic evaluation of health care .
	manualset3
86587	2	398574	13	NULL	NULL	0	NULL	 severity approach 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	His ` generalised fair innings approach ' on the one hand , and the severity approach on the other , are two ways of incorporating concerns for fairness in economic evaluation of health care .
	manualset3
86588	3	398574	13	NULL	NULL	0	NULL	two ways of incorporating concerns for fairness	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	His ` generalised fair innings approach ' on the one hand , and the severity approach on the other , are two ways of incorporating concerns for fairness in economic evaluation of health care .
	manualset3
86589	4	398574	13	NULL	NULL	0	NULL	economic evaluation of health care	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	His ` generalised fair innings approach ' on the one hand , and the severity approach on the other , are two ways of incorporating concerns for fairness in economic evaluation of health care .
	manualset3
86590	1	398575	13	NULL	NULL	NULL	NULL	serum creatine kinase ( CK ) level 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	His serum creatine kinase ( CK ) level was extremely elevated , and chest X-ray revealed bilateral hilar lymphadenopathy and small nodules in bilateral lung fields .
	manualset3
86591	2	398575	13	NULL	NULL	0	NULL	chest X-ray 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	His serum creatine kinase ( CK ) level was extremely elevated , and chest X-ray revealed bilateral hilar lymphadenopathy and small nodules in bilateral lung fields .
	manualset3
86592	3	398575	13	NULL	NULL	0	NULL	bilateral hilar lymphadenopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	His serum creatine kinase ( CK ) level was extremely elevated , and chest X-ray revealed bilateral hilar lymphadenopathy and small nodules in bilateral lung fields .
	manualset3
86593	4	398575	13	NULL	NULL	NULL	NULL	small nodules in bilateral lung fields	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	His serum creatine kinase ( CK ) level was extremely elevated , and chest X-ray revealed bilateral hilar lymphadenopathy and small nodules in bilateral lung fields .
	manualset3
86594	1	398576	13	NULL	NULL	0	NULL	theory of `` determinant spreading ''	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	His theory of `` determinant spreading '' is one of the cornerstones of our modern understanding of autoimmunity .
	manualset3
86595	2	398576	13	NULL	NULL	0	NULL	modern understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	His theory of `` determinant spreading '' is one of the cornerstones of our modern understanding of autoimmunity .
	manualset3
86596	3	398576	13	NULL	NULL	0	NULL	autoimmunity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	His theory of `` determinant spreading '' is one of the cornerstones of our modern understanding of autoimmunity .
	manualset3
86597	1	398577	13	NULL	NULL	0	NULL	young wife	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	His young wife presented him with a daughter Bianca , and a son Gaspare , but in 1861 she died , leaving him with the responsibility of rearing the children .
	manualset3
86598	2	398577	13	NULL	NULL	0	NULL	daughter Bianca	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	His young wife presented him with a daughter Bianca , and a son Gaspare , but in 1861 she died , leaving him with the responsibility of rearing the children .
	manualset3
86599	3	398577	13	NULL	NULL	0	NULL	son Gaspare	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	His young wife presented him with a daughter Bianca , and a son Gaspare , but in 1861 she died , leaving him with the responsibility of rearing the children .
	manualset3
86600	4	398577	13	NULL	NULL	0	NULL	1861	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	His young wife presented him with a daughter Bianca , and a son Gaspare , but in 1861 she died , leaving him with the responsibility of rearing the children .
	manualset3
86601	5	398577	13	NULL	NULL	0	NULL	died	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	His young wife presented him with a daughter Bianca , and a son Gaspare , but in 1861 she died , leaving him with the responsibility of rearing the children .
	manualset3
86602	6	398577	13	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	His young wife presented him with a daughter Bianca , and a son Gaspare , but in 1861 she died , leaving him with the responsibility of rearing the children .
	manualset3
86603	1	398578	13	NULL	NULL	0	NULL	His1	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	His1 and His2 are distantly related , spindle-shaped haloviruses belonging to the novel virus group , Salterprovirus .
	manualset3
86604	2	398578	13	NULL	NULL	0	NULL	His2	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	His1 and His2 are distantly related , spindle-shaped haloviruses belonging to the novel virus group , Salterprovirus .
	manualset3
86605	3	398578	13	NULL	NULL	0	NULL	spindle-shaped haloviruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	His1 and His2 are distantly related , spindle-shaped haloviruses belonging to the novel virus group , Salterprovirus .
	manualset3
86606	4	398578	13	NULL	NULL	0	NULL	novel virus group , Salterprovirus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	His1 and His2 are distantly related , spindle-shaped haloviruses belonging to the novel virus group , Salterprovirus .
	manualset3
86607	1	398579	13	NULL	NULL	0	NULL	His373 in flavocytochrome b2	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	His373 in flavocytochrome b2 has been proposed to act as an active site base during the oxidation of lactate to pyruvate , most likely by removing the lactate hydroxyl proton .
	manualset3
86608	2	398579	13	NULL	NULL	0	NULL	active site base	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	His373 in flavocytochrome b2 has been proposed to act as an active site base during the oxidation of lactate to pyruvate , most likely by removing the lactate hydroxyl proton .
	manualset3
86609	3	398579	13	NULL	NULL	0	NULL	 oxidation of lactate to pyruvate 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	His373 in flavocytochrome b2 has been proposed to act as an active site base during the oxidation of lactate to pyruvate , most likely by removing the lactate hydroxyl proton .
	manualset3
86610	4	398579	13	NULL	NULL	0	NULL	removing the lactate hydroxyl proton	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	His373 in flavocytochrome b2 has been proposed to act as an active site base during the oxidation of lactate to pyruvate , most likely by removing the lactate hydroxyl proton .
	manualset3
86611	1	398580	13	NULL	NULL	0	NULL	Terminology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Terminology and classification of automobile injuries ) .
	manualset3
86612	2	398580	13	NULL	NULL	0	NULL	classification	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Terminology and classification of automobile injuries ) .
	manualset3
86613	3	398580	13	NULL	NULL	0	NULL	automobile injuries	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Terminology and classification of automobile injuries ) .
	manualset3
86614	1	398581	13	NULL	NULL	0	NULL	Histamine-induced surface expression of P-selectin 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Histamine-induced surface expression of P-selectin was blocked by the histamine H2 receptor antagonist cimetidine .
	manualset3
86615	2	398581	13	NULL	NULL	0	NULL	histamine H2 receptor antagonist cimetidine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Histamine-induced surface expression of P-selectin was blocked by the histamine H2 receptor antagonist cimetidine .
	manualset3
86616	1	398582	13	NULL	NULL	0	NULL	Histamine release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Histamine release by the calcium ionophore ( A 23187 ) added to cells at intervals before the addition of calcium did not show significant decay .7 .
	manualset3
86617	2	398582	13	NULL	NULL	0	NULL	calcium ionophore ( A 23187 ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Histamine release by the calcium ionophore ( A 23187 ) added to cells at intervals before the addition of calcium did not show significant decay .7 .
	manualset3
86618	3	398582	13	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Histamine release by the calcium ionophore ( A 23187 ) added to cells at intervals before the addition of calcium did not show significant decay .7 .
	manualset3
86619	4	398582	13	NULL	NULL	0	NULL	intervals	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Histamine release by the calcium ionophore ( A 23187 ) added to cells at intervals before the addition of calcium did not show significant decay .7 .
	manualset3
86620	5	398582	13	NULL	NULL	NULL	NULL	calcium	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Histamine release by the calcium ionophore ( A 23187 ) added to cells at intervals before the addition of calcium did not show significant decay .7 .
	manualset3
86621	6	398582	13	NULL	NULL	0	NULL	significant decay .7	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histamine release by the calcium ionophore ( A 23187 ) added to cells at intervals before the addition of calcium did not show significant decay .7 .
	manualset3
86622	1	398583	13	NULL	NULL	0	NULL	Histidine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Histidine , which is known to activate motility of starfish sperm , also raised the ( pH ) i during the motility activation .
	manualset3
86623	2	398583	13	NULL	NULL	0	NULL	motility of starfish sperm	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Histidine , which is known to activate motility of starfish sperm , also raised the ( pH ) i during the motility activation .
	manualset3
86624	3	398583	13	NULL	NULL	NULL	NULL	( pH ) i 	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Histidine , which is known to activate motility of starfish sperm , also raised the ( pH ) i during the motility activation .
	manualset3
86625	4	398583	13	NULL	NULL	0	NULL	motility activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Histidine , which is known to activate motility of starfish sperm , also raised the ( pH ) i during the motility activation .
	manualset3
86626	1	398584	13	NULL	NULL	0	NULL	Histidine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Histidine and tryptamine also gave products upon UV irradiation that competed with TCDD .
	manualset3
86627	2	398584	13	NULL	NULL	0	NULL	tryptamine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Histidine and tryptamine also gave products upon UV irradiation that competed with TCDD .
	manualset3
86628	3	398584	13	NULL	NULL	0	NULL	UV irradiation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Histidine and tryptamine also gave products upon UV irradiation that competed with TCDD .
	manualset3
86629	4	398584	13	NULL	NULL	0	NULL	TCDD	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Histidine and tryptamine also gave products upon UV irradiation that competed with TCDD .
	manualset3
86630	1	398585	13	NULL	NULL	0	NULL	Histochemical changes 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Histochemical changes in enzymes of energy metabolism in the dentate gyrus accompany deafferentation and synaptic reorganization .
	manualset3
86631	2	398585	13	NULL	NULL	0	NULL	enzymes of energy metabolism	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Histochemical changes in enzymes of energy metabolism in the dentate gyrus accompany deafferentation and synaptic reorganization .
	manualset3
86632	3	398585	13	NULL	NULL	0	NULL	dentate gyrus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Histochemical changes in enzymes of energy metabolism in the dentate gyrus accompany deafferentation and synaptic reorganization .
	manualset3
86633	4	398585	13	NULL	NULL	0	NULL	deafferentation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Histochemical changes in enzymes of energy metabolism in the dentate gyrus accompany deafferentation and synaptic reorganization .
	manualset3
86634	5	398585	13	NULL	NULL	0	NULL	 synaptic reorganization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Histochemical changes in enzymes of energy metabolism in the dentate gyrus accompany deafferentation and synaptic reorganization .
	manualset3
86635	1	398586	13	NULL	NULL	0	NULL	Histochemical demonstration 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Histochemical demonstration of alpha-glucan phosphorylase activity in the human axillary apocrine sweat gland .
	manualset3
86636	2	398586	13	NULL	NULL	0	NULL	alpha-glucan phosphorylase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Histochemical demonstration of alpha-glucan phosphorylase activity in the human axillary apocrine sweat gland .
	manualset3
86637	3	398586	13	NULL	NULL	0	NULL	human axillary apocrine sweat gland	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Histochemical demonstration of alpha-glucan phosphorylase activity in the human axillary apocrine sweat gland .
	manualset3
86638	1	398587	13	NULL	NULL	0	NULL	Histocompatibility antigens	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Histocompatibility antigens on mouse spermatozoa .
	manualset3
86639	2	398587	13	NULL	NULL	0	NULL	mouse spermatozoa	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Histocompatibility antigens on mouse spermatozoa .
	manualset3
86640	1	398588	13	NULL	NULL	0	NULL	Association	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( The Association should be the information center ) .
	manualset3
86641	2	398588	13	NULL	NULL	0	NULL	 information center	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( The Association should be the information center ) .
	manualset3
86642	1	398589	13	NULL	NULL	0	NULL	Histologic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Histologic analysis demonstrated an intact endothelial surface in the stenotic segments , confirmed by the demonstration of factor VIII production by these cells .
	manualset3
86643	2	398589	13	NULL	NULL	0	NULL	intact endothelial surface in the stenotic segments	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histologic analysis demonstrated an intact endothelial surface in the stenotic segments , confirmed by the demonstration of factor VIII production by these cells .
	manualset3
86644	3	398589	13	NULL	NULL	NULL	NULL	 factor VIII production	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Histologic analysis demonstrated an intact endothelial surface in the stenotic segments , confirmed by the demonstration of factor VIII production by these cells .
	manualset3
86645	4	398589	13	NULL	NULL	0	NULL	 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Histologic analysis demonstrated an intact endothelial surface in the stenotic segments , confirmed by the demonstration of factor VIII production by these cells .
	manualset3
86646	1	398590	13	NULL	NULL	0	NULL	Histologic appearances of tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histologic appearances of tumors remained constant in subsequent passages .
	manualset3
86647	2	398590	13	NULL	NULL	0	NULL	subsequent passages	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Histologic appearances of tumors remained constant in subsequent passages .
	manualset3
86648	1	398591	13	NULL	NULL	0	NULL	Histologic evaluation of hepatic biopsy specimens	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Histologic evaluation of hepatic biopsy specimens from the 2 dogs revealed granulomatous hepatitis in the Basset Hound and lymphocytic hepatitis with fibrosis and copper accumulation in the Doberman Pinscher .
	manualset3
86650	3	398591	13	NULL	NULL	0	NULL	granulomatous hepatitis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Histologic evaluation of hepatic biopsy specimens from the 2 dogs revealed granulomatous hepatitis in the Basset Hound and lymphocytic hepatitis with fibrosis and copper accumulation in the Doberman Pinscher .
	manualset3
86651	4	398591	13	NULL	NULL	0	NULL	Basset Hound 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Histologic evaluation of hepatic biopsy specimens from the 2 dogs revealed granulomatous hepatitis in the Basset Hound and lymphocytic hepatitis with fibrosis and copper accumulation in the Doberman Pinscher .
	manualset3
86652	5	398591	13	NULL	NULL	0	NULL	lymphocytic hepatitis with fibrosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Histologic evaluation of hepatic biopsy specimens from the 2 dogs revealed granulomatous hepatitis in the Basset Hound and lymphocytic hepatitis with fibrosis and copper accumulation in the Doberman Pinscher .
	manualset3
86653	6	398591	13	NULL	NULL	0	NULL	copper accumulation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histologic evaluation of hepatic biopsy specimens from the 2 dogs revealed granulomatous hepatitis in the Basset Hound and lymphocytic hepatitis with fibrosis and copper accumulation in the Doberman Pinscher .
	manualset3
86654	7	398591	13	NULL	NULL	0	NULL	Doberman Pinscher	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Histologic evaluation of hepatic biopsy specimens from the 2 dogs revealed granulomatous hepatitis in the Basset Hound and lymphocytic hepatitis with fibrosis and copper accumulation in the Doberman Pinscher .
	manualset3
89565	8	398591	13	NULL	NULL	0	NULL	 2 dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Histologic evaluation of hepatic biopsy specimens from the 2 dogs revealed granulomatous hepatitis in the Basset Hound and lymphocytic hepatitis with fibrosis and copper accumulation in the Doberman Pinscher .
	manualset3
86649	1	398592	13	NULL	NULL	NULL	NULL	Histologic examination	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Histologic examination showed a histological pattern of interstitial granulomatous dermatitis .
	manualset3
86658	2	398592	13	NULL	NULL	NULL	NULL	histological pattern 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Histologic examination showed a histological pattern of interstitial granulomatous dermatitis .
	manualset3
86731	3	398592	13	NULL	NULL	0	NULL	interstitial granulomatous dermatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Histologic examination showed a histological pattern of interstitial granulomatous dermatitis .
	manualset3
86738	1	398593	13	NULL	NULL	0	NULL	Histologic examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Histologic examination showed that epididymal adipocyte size was smaller in mice fed the HF + 3 % CO. .
	manualset3
86740	2	398593	13	NULL	NULL	0	NULL	epididymal adipocyte	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Histologic examination showed that epididymal adipocyte size was smaller in mice fed the HF + 3 % CO. .
	manualset3
86741	3	398593	13	NULL	NULL	0	NULL	size	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Histologic examination showed that epididymal adipocyte size was smaller in mice fed the HF + 3 % CO. .
	manualset3
86743	4	398593	13	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Histologic examination showed that epididymal adipocyte size was smaller in mice fed the HF + 3 % CO. .
	manualset3
86744	5	398593	13	NULL	NULL	0	NULL	HF + 3 % CO	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Histologic examination showed that epididymal adipocyte size was smaller in mice fed the HF + 3 % CO. .
	manualset3
86746	1	398594	13	NULL	NULL	0	NULL	Histological analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological analysis of the aneurysm wall showed non-caseating granulomata .
	manualset3
86749	2	398594	13	NULL	NULL	0	NULL	aneurysm wall 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological analysis of the aneurysm wall showed non-caseating granulomata .
	manualset3
86750	3	398594	13	NULL	NULL	0	NULL	non-caseating granulomata	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological analysis of the aneurysm wall showed non-caseating granulomata .
	manualset3
86752	1	398595	13	NULL	NULL	0	NULL	Histological analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological analysis revealed well-differentiated HCC in both of the tumors .
	manualset3
86755	2	398595	13	NULL	NULL	0	NULL	well-differentiated HCC 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological analysis revealed well-differentiated HCC in both of the tumors .
	manualset3
86759	3	398595	13	NULL	NULL	NULL	NULL	tumors	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Histological analysis revealed well-differentiated HCC in both of the tumors .
	manualset3
86765	1	398596	13	NULL	NULL	0	NULL	Histological and immunocytochemical studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological and immunocytochemical studies showed good survival of both PN and VM grafts .
	manualset3
86766	2	398596	13	NULL	NULL	NULL	NULL	good survival	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Histological and immunocytochemical studies showed good survival of both PN and VM grafts .
	manualset3
86771	3	398596	13	NULL	NULL	0	NULL	PN grafts	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological and immunocytochemical studies showed good survival of both PN and VM grafts .
	manualset3
86772	4	398596	13	NULL	NULL	0	NULL	 VM grafts	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological and immunocytochemical studies showed good survival of both PN and VM grafts .
	manualset3
86776	1	398597	13	NULL	NULL	0	NULL	Histological changes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological changes in bladders of patients submitted to ifosfamide chemotherapy even with mesna prophylaxis .
	manualset3
86777	2	398597	13	NULL	NULL	NULL	NULL	bladders	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Histological changes in bladders of patients submitted to ifosfamide chemotherapy even with mesna prophylaxis .
	manualset3
86778	4	398597	13	NULL	NULL	NULL	NULL	ifosfamide chemotherapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Histological changes in bladders of patients submitted to ifosfamide chemotherapy even with mesna prophylaxis .
	manualset3
86781	5	398597	13	NULL	NULL	NULL	NULL	mesna prophylaxis 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Histological changes in bladders of patients submitted to ifosfamide chemotherapy even with mesna prophylaxis .
	manualset3
86782	3	398597	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological changes in bladders of patients submitted to ifosfamide chemotherapy even with mesna prophylaxis .
	manualset3
86785	1	398598	13	NULL	NULL	0	NULL	Histological diagnosis of the lesions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological diagnosis of the lesions revealed : astrocytomas in 14 patients , oligodendroglioma in one , ependymoma in one , arteriovenous malformations in two , radionecrosis in one , cryptococcal abscess in one , demyelinating disease in three , and infarctions in three .
	manualset3
86786	2	398598	13	NULL	NULL	0	NULL	astrocytomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological diagnosis of the lesions revealed : astrocytomas in 14 patients , oligodendroglioma in one , ependymoma in one , arteriovenous malformations in two , radionecrosis in one , cryptococcal abscess in one , demyelinating disease in three , and infarctions in three .
	manualset3
86788	3	398598	13	NULL	NULL	0	NULL	14 patients	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological diagnosis of the lesions revealed : astrocytomas in 14 patients , oligodendroglioma in one , ependymoma in one , arteriovenous malformations in two , radionecrosis in one , cryptococcal abscess in one , demyelinating disease in three , and infarctions in three .
	manualset3
86789	4	398598	13	NULL	NULL	0	NULL	oligodendroglioma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological diagnosis of the lesions revealed : astrocytomas in 14 patients , oligodendroglioma in one , ependymoma in one , arteriovenous malformations in two , radionecrosis in one , cryptococcal abscess in one , demyelinating disease in three , and infarctions in three .
	manualset3
86790	5	398598	13	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological diagnosis of the lesions revealed : astrocytomas in 14 patients , oligodendroglioma in one , ependymoma in one , arteriovenous malformations in two , radionecrosis in one , cryptococcal abscess in one , demyelinating disease in three , and infarctions in three .
	manualset3
86791	6	398598	13	NULL	NULL	0	NULL	 ependymoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological diagnosis of the lesions revealed : astrocytomas in 14 patients , oligodendroglioma in one , ependymoma in one , arteriovenous malformations in two , radionecrosis in one , cryptococcal abscess in one , demyelinating disease in three , and infarctions in three .
	manualset3
86792	7	398598	13	NULL	NULL	0	NULL	one 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological diagnosis of the lesions revealed : astrocytomas in 14 patients , oligodendroglioma in one , ependymoma in one , arteriovenous malformations in two , radionecrosis in one , cryptococcal abscess in one , demyelinating disease in three , and infarctions in three .
	manualset3
86793	8	398598	13	NULL	NULL	0	NULL	arteriovenous malformations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological diagnosis of the lesions revealed : astrocytomas in 14 patients , oligodendroglioma in one , ependymoma in one , arteriovenous malformations in two , radionecrosis in one , cryptococcal abscess in one , demyelinating disease in three , and infarctions in three .
	manualset3
86794	9	398598	13	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological diagnosis of the lesions revealed : astrocytomas in 14 patients , oligodendroglioma in one , ependymoma in one , arteriovenous malformations in two , radionecrosis in one , cryptococcal abscess in one , demyelinating disease in three , and infarctions in three .
	manualset3
86796	10	398598	13	NULL	NULL	0	NULL	radionecrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological diagnosis of the lesions revealed : astrocytomas in 14 patients , oligodendroglioma in one , ependymoma in one , arteriovenous malformations in two , radionecrosis in one , cryptococcal abscess in one , demyelinating disease in three , and infarctions in three .
	manualset3
86797	11	398598	13	NULL	NULL	0	NULL	 one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological diagnosis of the lesions revealed : astrocytomas in 14 patients , oligodendroglioma in one , ependymoma in one , arteriovenous malformations in two , radionecrosis in one , cryptococcal abscess in one , demyelinating disease in three , and infarctions in three .
	manualset3
86799	12	398598	13	NULL	NULL	0	NULL	cryptococcal abscess	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological diagnosis of the lesions revealed : astrocytomas in 14 patients , oligodendroglioma in one , ependymoma in one , arteriovenous malformations in two , radionecrosis in one , cryptococcal abscess in one , demyelinating disease in three , and infarctions in three .
	manualset3
86800	13	398598	13	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological diagnosis of the lesions revealed : astrocytomas in 14 patients , oligodendroglioma in one , ependymoma in one , arteriovenous malformations in two , radionecrosis in one , cryptococcal abscess in one , demyelinating disease in three , and infarctions in three .
	manualset3
86802	14	398598	13	NULL	NULL	0	NULL	demyelinating disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological diagnosis of the lesions revealed : astrocytomas in 14 patients , oligodendroglioma in one , ependymoma in one , arteriovenous malformations in two , radionecrosis in one , cryptococcal abscess in one , demyelinating disease in three , and infarctions in three .
	manualset3
86803	15	398598	13	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological diagnosis of the lesions revealed : astrocytomas in 14 patients , oligodendroglioma in one , ependymoma in one , arteriovenous malformations in two , radionecrosis in one , cryptococcal abscess in one , demyelinating disease in three , and infarctions in three .
	manualset3
86804	16	398598	13	NULL	NULL	0	NULL	infarctions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological diagnosis of the lesions revealed : astrocytomas in 14 patients , oligodendroglioma in one , ependymoma in one , arteriovenous malformations in two , radionecrosis in one , cryptococcal abscess in one , demyelinating disease in three , and infarctions in three .
	manualset3
86806	17	398598	13	NULL	NULL	0	NULL	three 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological diagnosis of the lesions revealed : astrocytomas in 14 patients , oligodendroglioma in one , ependymoma in one , arteriovenous malformations in two , radionecrosis in one , cryptococcal abscess in one , demyelinating disease in three , and infarctions in three .
	manualset3
86809	1	398599	13	NULL	NULL	0	NULL	Analysis of late components	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Analysis of late components of evoked potentials arising in the paramedian lobule of the cerebellum in response to stimulation of nerves and the cerebral cortex ) .
	manualset3
86810	2	398599	13	NULL	NULL	0	NULL	evoked potentials 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Analysis of late components of evoked potentials arising in the paramedian lobule of the cerebellum in response to stimulation of nerves and the cerebral cortex ) .
	manualset3
86811	3	398599	13	NULL	NULL	0	NULL	paramedian lobule of the cerebellum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Analysis of late components of evoked potentials arising in the paramedian lobule of the cerebellum in response to stimulation of nerves and the cerebral cortex ) .
	manualset3
86812	4	398599	13	NULL	NULL	0	NULL	stimulation of nerves	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Analysis of late components of evoked potentials arising in the paramedian lobule of the cerebellum in response to stimulation of nerves and the cerebral cortex ) .
	manualset3
86813	5	398599	13	NULL	NULL	0	NULL	cerebral cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Analysis of late components of evoked potentials arising in the paramedian lobule of the cerebellum in response to stimulation of nerves and the cerebral cortex ) .
	manualset3
86814	1	398600	13	NULL	NULL	0	NULL	C-cell system of the thyroid	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	( The C-cell system of the thyroid in rats following a flight on the Kosmos 1667 biosatellite ) .
	manualset3
86815	2	398600	13	NULL	NULL	0	NULL	rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( The C-cell system of the thyroid in rats following a flight on the Kosmos 1667 biosatellite ) .
	manualset3
86816	3	398600	13	NULL	NULL	0	NULL	Kosmos 1667 biosatellite	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( The C-cell system of the thyroid in rats following a flight on the Kosmos 1667 biosatellite ) .
	manualset3
86818	1	398601	13	NULL	NULL	0	NULL	Histological examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological examination demonstrated bladder endometriosis sparing the urothelium .
	manualset3
86819	2	398601	13	NULL	NULL	0	NULL	bladder endometriosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological examination demonstrated bladder endometriosis sparing the urothelium .
	manualset3
86820	3	398601	13	NULL	NULL	0	NULL	urothelium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological examination demonstrated bladder endometriosis sparing the urothelium .
	manualset3
86821	1	398602	13	NULL	NULL	0	NULL	Histological lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological lesions comprised of fragmentation of elastic fibers as well as extensive loss of elastic layers .
	manualset3
86822	2	398602	13	NULL	NULL	NULL	NULL	fragmentation of elastic fibers	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Histological lesions comprised of fragmentation of elastic fibers as well as extensive loss of elastic layers .
	manualset3
86823	3	398602	13	NULL	NULL	0	NULL	extensive loss of elastic layers	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological lesions comprised of fragmentation of elastic fibers as well as extensive loss of elastic layers .
	manualset3
86824	1	398603	13	NULL	NULL	0	NULL	Histological studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological studies and TEM revealed that Y. enterocolitica selectively invaded the PP via M cells but not via other cells of the FAE .
	manualset3
86825	2	398603	13	NULL	NULL	0	NULL	TEM	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological studies and TEM revealed that Y. enterocolitica selectively invaded the PP via M cells but not via other cells of the FAE .
	manualset3
86826	3	398603	13	NULL	NULL	0	NULL	Y. enterocolitica 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological studies and TEM revealed that Y. enterocolitica selectively invaded the PP via M cells but not via other cells of the FAE .
	manualset3
86827	4	398603	13	NULL	NULL	0	NULL	PP	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological studies and TEM revealed that Y. enterocolitica selectively invaded the PP via M cells but not via other cells of the FAE .
	manualset3
86828	5	398603	13	NULL	NULL	0	NULL	M cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological studies and TEM revealed that Y. enterocolitica selectively invaded the PP via M cells but not via other cells of the FAE .
	manualset3
86829	6	398603	13	NULL	NULL	0	NULL	other cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological studies and TEM revealed that Y. enterocolitica selectively invaded the PP via M cells but not via other cells of the FAE .
	manualset3
86830	7	398603	13	NULL	NULL	0	NULL	FAE 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological studies and TEM revealed that Y. enterocolitica selectively invaded the PP via M cells but not via other cells of the FAE .
	manualset3
86831	1	398604	13	NULL	NULL	0	NULL	tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histologically , tumors were classified as MALT-type lymphoma .
	manualset3
86832	2	398604	13	NULL	NULL	0	NULL	MALT-type lymphoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Histologically , tumors were classified as MALT-type lymphoma .
	manualset3
86833	1	398605	13	NULL	NULL	0	NULL	Histology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Histology revealed fibrocystic change in 66 , fibroadenoma in 27 , radial scar/complex sclerosing lesion in 23 , atypical ductal hyperplasia only in eight , and a variety of unusual benign lesions in 13 .
	manualset3
86834	2	398605	13	NULL	NULL	0	NULL	fibrocystic change	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histology revealed fibrocystic change in 66 , fibroadenoma in 27 , radial scar/complex sclerosing lesion in 23 , atypical ductal hyperplasia only in eight , and a variety of unusual benign lesions in 13 .
	manualset3
86835	3	398605	13	NULL	NULL	0	NULL	66	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Histology revealed fibrocystic change in 66 , fibroadenoma in 27 , radial scar/complex sclerosing lesion in 23 , atypical ductal hyperplasia only in eight , and a variety of unusual benign lesions in 13 .
	manualset3
86836	4	398605	13	NULL	NULL	0	NULL	fibroadenoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histology revealed fibrocystic change in 66 , fibroadenoma in 27 , radial scar/complex sclerosing lesion in 23 , atypical ductal hyperplasia only in eight , and a variety of unusual benign lesions in 13 .
	manualset3
86837	5	398605	13	NULL	NULL	0	NULL	27	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histology revealed fibrocystic change in 66 , fibroadenoma in 27 , radial scar/complex sclerosing lesion in 23 , atypical ductal hyperplasia only in eight , and a variety of unusual benign lesions in 13 .
	manualset3
86838	6	398605	13	NULL	NULL	0	NULL	radial scar/complex sclerosing lesion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histology revealed fibrocystic change in 66 , fibroadenoma in 27 , radial scar/complex sclerosing lesion in 23 , atypical ductal hyperplasia only in eight , and a variety of unusual benign lesions in 13 .
	manualset3
86839	7	398605	13	NULL	NULL	0	NULL	23	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Histology revealed fibrocystic change in 66 , fibroadenoma in 27 , radial scar/complex sclerosing lesion in 23 , atypical ductal hyperplasia only in eight , and a variety of unusual benign lesions in 13 .
	manualset3
86840	8	398605	13	NULL	NULL	0	NULL	atypical ductal hyperplasia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histology revealed fibrocystic change in 66 , fibroadenoma in 27 , radial scar/complex sclerosing lesion in 23 , atypical ductal hyperplasia only in eight , and a variety of unusual benign lesions in 13 .
	manualset3
86841	9	398605	13	NULL	NULL	0	NULL	eight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Histology revealed fibrocystic change in 66 , fibroadenoma in 27 , radial scar/complex sclerosing lesion in 23 , atypical ductal hyperplasia only in eight , and a variety of unusual benign lesions in 13 .
	manualset3
86842	10	398605	13	NULL	NULL	0	NULL	variety of unusual benign lesions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histology revealed fibrocystic change in 66 , fibroadenoma in 27 , radial scar/complex sclerosing lesion in 23 , atypical ductal hyperplasia only in eight , and a variety of unusual benign lesions in 13 .
	manualset3
86843	11	398605	13	NULL	NULL	0	NULL	13	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Histology revealed fibrocystic change in 66 , fibroadenoma in 27 , radial scar/complex sclerosing lesion in 23 , atypical ductal hyperplasia only in eight , and a variety of unusual benign lesions in 13 .
	manualset3
86844	1	398606	13	NULL	NULL	0	NULL	Histone acetyltransferases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Histone acetyltransferases as regulators of nonhistone proteins : the role of interferon regulatory factor acetylation on gene transcription .
	manualset3
86845	2	398606	13	NULL	NULL	0	NULL	regulators of nonhistone proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Histone acetyltransferases as regulators of nonhistone proteins : the role of interferon regulatory factor acetylation on gene transcription .
	manualset3
86846	3	398606	13	NULL	NULL	0	NULL	interferon regulatory factor acetylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Histone acetyltransferases as regulators of nonhistone proteins : the role of interferon regulatory factor acetylation on gene transcription .
	manualset3
86847	4	398606	13	NULL	NULL	0	NULL	gene transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Histone acetyltransferases as regulators of nonhistone proteins : the role of interferon regulatory factor acetylation on gene transcription .
	manualset3
86848	1	398607	13	NULL	NULL	0	NULL	Histone deacetylase ( HDAC ) inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Histone deacetylase ( HDAC ) inhibitors attenuate cardiac hypertrophy by suppressing autophagy .
	manualset3
86849	2	398607	13	NULL	NULL	0	NULL	cardiac hypertrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histone deacetylase ( HDAC ) inhibitors attenuate cardiac hypertrophy by suppressing autophagy .
	manualset3
86850	3	398607	13	NULL	NULL	0	NULL	autophagy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Histone deacetylase ( HDAC ) inhibitors attenuate cardiac hypertrophy by suppressing autophagy .
	manualset3
86851	1	398608	13	NULL	NULL	0	NULL	Histone deacetylase inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Histone deacetylase inhibitors decrease DNA methyltransferase-3B messenger RNA stability and down-regulate de novo DNA methyltransferase activity in human endometrial cells .
	manualset3
86852	2	398608	13	NULL	NULL	0	NULL	DNA methyltransferase-3B messenger RNA stability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Histone deacetylase inhibitors decrease DNA methyltransferase-3B messenger RNA stability and down-regulate de novo DNA methyltransferase activity in human endometrial cells .
	manualset3
86853	3	398608	13	NULL	NULL	0	NULL	de novo DNA methyltransferase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Histone deacetylase inhibitors decrease DNA methyltransferase-3B messenger RNA stability and down-regulate de novo DNA methyltransferase activity in human endometrial cells .
	manualset3
86854	4	398608	13	NULL	NULL	0	NULL	 human endometrial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Histone deacetylase inhibitors decrease DNA methyltransferase-3B messenger RNA stability and down-regulate de novo DNA methyltransferase activity in human endometrial cells .
	manualset3
86855	1	398609	13	NULL	NULL	0	NULL	Histopathologic examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Histopathologic examination confirmed that excision of the tumor was complete .
	manualset3
86856	2	398609	13	NULL	NULL	0	NULL	excision of the tumor was complete	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histopathologic examination confirmed that excision of the tumor was complete .
	manualset3
86857	1	398610	13	NULL	NULL	0	NULL	Histopathologic studies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Histopathologic studies indicate that laminitis is associated with changes of the vasculature .
	manualset3
86858	2	398610	13	NULL	NULL	0	NULL	laminitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Histopathologic studies indicate that laminitis is associated with changes of the vasculature .
	manualset3
86859	3	398610	13	NULL	NULL	0	NULL	changes of the vasculature	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histopathologic studies indicate that laminitis is associated with changes of the vasculature .
	manualset3
86860	1	398611	13	NULL	NULL	0	NULL	Histopathological analysis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Histopathological analysis established the diagnosis as peritoneal pseudomyxoma .
	manualset3
86861	2	398611	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Histopathological analysis established the diagnosis as peritoneal pseudomyxoma .
	manualset3
86862	3	398611	13	NULL	NULL	0	NULL	peritoneal pseudomyxoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Histopathological analysis established the diagnosis as peritoneal pseudomyxoma .
	manualset3
86863	1	398612	13	NULL	NULL	NULL	NULL	Histopathological changes 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Histopathological changes in the bile - or acid-perfused esophagus were consistent with the findings associated with reflux esophagitis .
	manualset3
86864	3	398612	13	NULL	NULL	NULL	NULL	findings	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Histopathological changes in the bile - or acid-perfused esophagus were consistent with the findings associated with reflux esophagitis .
	manualset3
86865	4	398612	13	NULL	NULL	NULL	NULL	reflux esophagitis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Histopathological changes in the bile - or acid-perfused esophagus were consistent with the findings associated with reflux esophagitis .
	manualset3
86866	2	398612	13	NULL	NULL	0	NULL	bile - or acid-perfused esophagus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Histopathological changes in the bile - or acid-perfused esophagus were consistent with the findings associated with reflux esophagitis .
	manualset3
86867	1	398613	13	NULL	NULL	NULL	NULL	Histopathological examination	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Histopathological examination of the tumor indicated well differentiated adenocarcinoma compatible with the metastasis from the previous descending colon cancer .
	manualset3
86868	2	398613	13	NULL	NULL	0	NULL	tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histopathological examination of the tumor indicated well differentiated adenocarcinoma compatible with the metastasis from the previous descending colon cancer .
	manualset3
86869	3	398613	13	NULL	NULL	0	NULL	well differentiated adenocarcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Histopathological examination of the tumor indicated well differentiated adenocarcinoma compatible with the metastasis from the previous descending colon cancer .
	manualset3
86870	4	398613	13	NULL	NULL	0	NULL	metastasis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Histopathological examination of the tumor indicated well differentiated adenocarcinoma compatible with the metastasis from the previous descending colon cancer .
	manualset3
86871	5	398613	13	NULL	NULL	0	NULL	descending colon cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Histopathological examination of the tumor indicated well differentiated adenocarcinoma compatible with the metastasis from the previous descending colon cancer .
	manualset3
86872	1	398614	13	NULL	NULL	0	NULL	Histopathological studies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Histopathological studies proved the tissue compatibility of ALOME to be safe .
	manualset3
86873	2	398614	13	NULL	NULL	0	NULL	 tissue compatibility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histopathological studies proved the tissue compatibility of ALOME to be safe .
	manualset3
86874	3	398614	13	NULL	NULL	0	NULL	ALOME	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Histopathological studies proved the tissue compatibility of ALOME to be safe .
	manualset3
86875	4	398614	13	NULL	NULL	0	NULL	 safe	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histopathological studies proved the tissue compatibility of ALOME to be safe .
	manualset3
86876	1	398615	13	NULL	NULL	0	NULL	Histopathology and cell proliferation analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Histopathology and cell proliferation analysis demonstrated a compound - and sex-specific onset of preneoplastic lesions .
	manualset3
86877	2	398615	13	NULL	NULL	NULL	NULL	compound - and sex-specific onset of preneoplastic lesions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Histopathology and cell proliferation analysis demonstrated a compound - and sex-specific onset of preneoplastic lesions .
	manualset3
86879	1	398616	13	NULL	NULL	0	NULL	role of Ca ( 2 + ) signals	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Historically , much of the research effort in this area has focused on the role of Ca ( 2 + ) signals in cell-cycle progression .
	manualset3
86880	2	398616	13	NULL	NULL	NULL	NULL	cell-cycle progression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Historically , much of the research effort in this area has focused on the role of Ca ( 2 + ) signals in cell-cycle progression .
	manualset3
86936	3	398616	13	NULL	NULL	0	NULL	research effort 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Historically , much of the research effort in this area has focused on the role of Ca ( 2 + ) signals in cell-cycle progression .
	manualset3
86881	1	398617	13	NULL	NULL	NULL	NULL	History of pathology	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	History of pathology in California .
	manualset3
86882	2	398617	13	NULL	NULL	0	NULL	California	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	History of pathology in California .
	manualset3
86883	1	398618	13	NULL	NULL	NULL	NULL	History of risk factors	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	History of risk factors , especially of snoring and sleeping habits was recorded with structured questionnaire during interview .
	manualset3
86884	2	398618	13	NULL	NULL	0	NULL	snoring and sleeping habits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	History of risk factors , especially of snoring and sleeping habits was recorded with structured questionnaire during interview .
	manualset3
86885	3	398618	13	NULL	NULL	0	NULL	structured questionnaire during interview	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	History of risk factors , especially of snoring and sleeping habits was recorded with structured questionnaire during interview .
	manualset3
86886	1	398619	13	NULL	NULL	0	NULL	Hodgkin lymphoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hodgkin lymphoma in temporal association with growth hormone replacement .
	manualset3
86887	2	398619	13	NULL	NULL	0	NULL	temporal association 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hodgkin lymphoma in temporal association with growth hormone replacement .
	manualset3
86888	3	398619	13	NULL	NULL	0	NULL	growth hormone replacement	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hodgkin lymphoma in temporal association with growth hormone replacement .
	manualset3
86889	1	398620	13	NULL	NULL	0	NULL	Hoffman 's plastic lymphangitis of the penis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hoffman 's plastic lymphangitis of the penis is a benign , uncommon entity whose aetiology is still unknown .
	manualset3
86890	2	398620	13	NULL	NULL	0	NULL	benign	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hoffman 's plastic lymphangitis of the penis is a benign , uncommon entity whose aetiology is still unknown .
	manualset3
86891	3	398620	13	NULL	NULL	0	NULL	aetiology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Hoffman 's plastic lymphangitis of the penis is a benign , uncommon entity whose aetiology is still unknown .
	manualset3
86892	1	398621	13	NULL	NULL	NULL	NULL	Home-based intervention	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Home-based intervention has been shown to provide long-term cost benefit in a range of chronic illnesses ; however , the role of home visits by respiratory therapists ( RT ) in COPD management has not been evaluated .
	manualset3
86893	2	398621	13	NULL	NULL	NULL	NULL	range of chronic illnesses	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Home-based intervention has been shown to provide long-term cost benefit in a range of chronic illnesses ; however , the role of home visits by respiratory therapists ( RT ) in COPD management has not been evaluated .
	manualset3
86894	3	398621	13	NULL	NULL	0	NULL	home visits by respiratory therapists ( RT )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Home-based intervention has been shown to provide long-term cost benefit in a range of chronic illnesses ; however , the role of home visits by respiratory therapists ( RT ) in COPD management has not been evaluated .
	manualset3
86895	4	398621	13	NULL	NULL	0	NULL	COPD management 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Home-based intervention has been shown to provide long-term cost benefit in a range of chronic illnesses ; however , the role of home visits by respiratory therapists ( RT ) in COPD management has not been evaluated .
	manualset3
86896	1	398622	13	NULL	NULL	0	NULL	Home care company	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Home care company is single source for purchase of epoprostenol .
	manualset3
86897	2	398622	13	NULL	NULL	0	NULL	single source for purchase	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Home care company is single source for purchase of epoprostenol .
	manualset3
86898	3	398622	13	NULL	NULL	0	NULL	epoprostenol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Home care company is single source for purchase of epoprostenol .
	manualset3
86899	1	398623	13	NULL	NULL	0	NULL	Home health aides 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Home health aides were offered to half of a group of 227 low-income diabetic clinic patients ; in the group offered aides , fasting blood sugar ( FBS ) declined when compared to control group ( 10.1 mg/dl vs an increase of 5.1 mg/dl ) , and missed clinic appointments and emergency room use also decreased .
	manualset3
86900	2	398623	13	NULL	NULL	0	NULL	half of a group of 227	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Home health aides were offered to half of a group of 227 low-income diabetic clinic patients ; in the group offered aides , fasting blood sugar ( FBS ) declined when compared to control group ( 10.1 mg/dl vs an increase of 5.1 mg/dl ) , and missed clinic appointments and emergency room use also decreased .
	manualset3
86901	3	398623	13	NULL	NULL	0	NULL	low-income diabetic clinic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Home health aides were offered to half of a group of 227 low-income diabetic clinic patients ; in the group offered aides , fasting blood sugar ( FBS ) declined when compared to control group ( 10.1 mg/dl vs an increase of 5.1 mg/dl ) , and missed clinic appointments and emergency room use also decreased .
	manualset3
86902	4	398623	13	NULL	NULL	0	NULL	group offered aides	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Home health aides were offered to half of a group of 227 low-income diabetic clinic patients ; in the group offered aides , fasting blood sugar ( FBS ) declined when compared to control group ( 10.1 mg/dl vs an increase of 5.1 mg/dl ) , and missed clinic appointments and emergency room use also decreased .
	manualset3
86903	5	398623	13	NULL	NULL	0	NULL	fasting blood sugar ( FBS ) declined	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Home health aides were offered to half of a group of 227 low-income diabetic clinic patients ; in the group offered aides , fasting blood sugar ( FBS ) declined when compared to control group ( 10.1 mg/dl vs an increase of 5.1 mg/dl ) , and missed clinic appointments and emergency room use also decreased .
	manualset3
86904	6	398623	13	NULL	NULL	0	NULL	control group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Home health aides were offered to half of a group of 227 low-income diabetic clinic patients ; in the group offered aides , fasting blood sugar ( FBS ) declined when compared to control group ( 10.1 mg/dl vs an increase of 5.1 mg/dl ) , and missed clinic appointments and emergency room use also decreased .
	manualset3
86905	7	398623	13	NULL	NULL	0	NULL	10.1 mg/dl vs an increase of 5.1 mg/dl 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Home health aides were offered to half of a group of 227 low-income diabetic clinic patients ; in the group offered aides , fasting blood sugar ( FBS ) declined when compared to control group ( 10.1 mg/dl vs an increase of 5.1 mg/dl ) , and missed clinic appointments and emergency room use also decreased .
	manualset3
86906	8	398623	13	NULL	NULL	0	NULL	clinic appointments	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Home health aides were offered to half of a group of 227 low-income diabetic clinic patients ; in the group offered aides , fasting blood sugar ( FBS ) declined when compared to control group ( 10.1 mg/dl vs an increase of 5.1 mg/dl ) , and missed clinic appointments and emergency room use also decreased .
	manualset3
86907	9	398623	13	NULL	NULL	0	NULL	emergency room	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Home health aides were offered to half of a group of 227 low-income diabetic clinic patients ; in the group offered aides , fasting blood sugar ( FBS ) declined when compared to control group ( 10.1 mg/dl vs an increase of 5.1 mg/dl ) , and missed clinic appointments and emergency room use also decreased .
	manualset3
86908	1	398624	13	NULL	NULL	0	NULL	Home visits	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Home visits were also conducted after discharge to assess the home care environment and give instant consultation , providing holistic health care with sustained quality of care .
	manualset3
86909	2	398624	13	NULL	NULL	0	NULL	discharge	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Home visits were also conducted after discharge to assess the home care environment and give instant consultation , providing holistic health care with sustained quality of care .
	manualset3
86910	3	398624	13	NULL	NULL	0	NULL	home care environment 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Home visits were also conducted after discharge to assess the home care environment and give instant consultation , providing holistic health care with sustained quality of care .
	manualset3
86911	4	398624	13	NULL	NULL	0	NULL	 instant consultation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Home visits were also conducted after discharge to assess the home care environment and give instant consultation , providing holistic health care with sustained quality of care .
	manualset3
86912	5	398624	13	NULL	NULL	NULL	NULL	holistic health care 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Home visits were also conducted after discharge to assess the home care environment and give instant consultation , providing holistic health care with sustained quality of care .
	manualset3
86913	6	398624	13	NULL	NULL	0	NULL	sustained quality of care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Home visits were also conducted after discharge to assess the home care environment and give instant consultation , providing holistic health care with sustained quality of care .
	manualset3
86914	1	398625	13	NULL	NULL	0	NULL	Homeowner attitudes	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Homeowner attitudes and practices towards residential landscape management in ohio , USA .
	manualset3
86915	2	398625	13	NULL	NULL	0	NULL	practices	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Homeowner attitudes and practices towards residential landscape management in ohio , USA .
	manualset3
86916	3	398625	13	NULL	NULL	0	NULL	residential landscape management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Homeowner attitudes and practices towards residential landscape management in ohio , USA .
	manualset3
86917	4	398625	13	NULL	NULL	0	NULL	ohio , USA	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Homeowner attitudes and practices towards residential landscape management in ohio , USA .
	manualset3
86918	1	398626	13	NULL	NULL	0	NULL	mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Homing in on mechanisms linking breast density to breast cancer risk .
	manualset3
86919	2	398626	13	NULL	NULL	0	NULL	breast density	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Homing in on mechanisms linking breast density to breast cancer risk .
	manualset3
86920	3	398626	13	NULL	NULL	0	NULL	breast cancer risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Homing in on mechanisms linking breast density to breast cancer risk .
	manualset3
86921	1	398627	13	NULL	NULL	0	NULL	Homocysteine levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Homocysteine levels and coronary heart disease in Syria .
	manualset3
86922	2	398627	13	NULL	NULL	0	NULL	coronary heart disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Homocysteine levels and coronary heart disease in Syria .
	manualset3
86923	3	398627	13	NULL	NULL	0	NULL	Syria	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Homocysteine levels and coronary heart disease in Syria .
	manualset3
86924	1	398628	13	NULL	NULL	0	NULL	Homogenous glycine receptor expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Homogenous glycine receptor expression in cortical plate neurons and Cajal-Retzius cells of neonatal rat cerebral cortex .
	manualset3
86925	2	398628	13	NULL	NULL	0	NULL	cortical plate neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Homogenous glycine receptor expression in cortical plate neurons and Cajal-Retzius cells of neonatal rat cerebral cortex .
	manualset3
86926	3	398628	13	NULL	NULL	0	NULL	Cajal-Retzius cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Homogenous glycine receptor expression in cortical plate neurons and Cajal-Retzius cells of neonatal rat cerebral cortex .
	manualset3
86927	4	398628	13	NULL	NULL	0	NULL	neonatal rat cerebral cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Homogenous glycine receptor expression in cortical plate neurons and Cajal-Retzius cells of neonatal rat cerebral cortex .
	manualset3
86928	1	398629	13	NULL	NULL	0	NULL	Homologous recombination	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Homologous recombination is a conserved molecular process that has primarily evolved for the repair of double-stranded DNA breaks and stalled replication forks .
	manualset3
86929	2	398629	13	NULL	NULL	0	NULL	molecular process	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Homologous recombination is a conserved molecular process that has primarily evolved for the repair of double-stranded DNA breaks and stalled replication forks .
	manualset3
86930	3	398629	13	NULL	NULL	NULL	NULL	repair of double-stranded DNA breaks	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Homologous recombination is a conserved molecular process that has primarily evolved for the repair of double-stranded DNA breaks and stalled replication forks .
	manualset3
86931	4	398629	13	NULL	NULL	0	NULL	stalled replication forks	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Homologous recombination is a conserved molecular process that has primarily evolved for the repair of double-stranded DNA breaks and stalled replication forks .
	manualset3
86932	1	398630	13	NULL	NULL	0	NULL	Homologous transient transfection experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Homologous transient transfection experiments were conducted employing a 0.9-kb fragment of the 5 ' flanking region of the human CRH gene coupled to the luciferase reporter gene , using Ishikawa human endometrial cells .
	manualset3
86933	2	398630	13	NULL	NULL	NULL	NULL	 0.9-kb fragment of the 5 ' flanking region of the human CRH gene	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Homologous transient transfection experiments were conducted employing a 0.9-kb fragment of the 5 ' flanking region of the human CRH gene coupled to the luciferase reporter gene , using Ishikawa human endometrial cells .
	manualset3
86934	3	398630	13	NULL	NULL	0	NULL	luciferase reporter gene	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Homologous transient transfection experiments were conducted employing a 0.9-kb fragment of the 5 ' flanking region of the human CRH gene coupled to the luciferase reporter gene , using Ishikawa human endometrial cells .
	manualset3
86935	4	398630	13	NULL	NULL	0	NULL	Ishikawa human endometrial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Homologous transient transfection experiments were conducted employing a 0.9-kb fragment of the 5 ' flanking region of the human CRH gene coupled to the luciferase reporter gene , using Ishikawa human endometrial cells .
	manualset3
86999	1	398631	13	NULL	NULL	0	NULL	Homologs 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Homologs of the recently described mouse pro genes , that transfer sensitivity to promotion of neoplastic transformation by tumor promoters , have been cloned from a genomic library of the human nasopharyngeal carcinoma ( NPC ) cell line CNE2 .
	manualset3
87000	2	398631	13	NULL	NULL	0	NULL	mouse pro genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Homologs of the recently described mouse pro genes , that transfer sensitivity to promotion of neoplastic transformation by tumor promoters , have been cloned from a genomic library of the human nasopharyngeal carcinoma ( NPC ) cell line CNE2 .
	manualset3
87001	3	398631	13	NULL	NULL	NULL	NULL	neoplastic transformation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Homologs of the recently described mouse pro genes , that transfer sensitivity to promotion of neoplastic transformation by tumor promoters , have been cloned from a genomic library of the human nasopharyngeal carcinoma ( NPC ) cell line CNE2 .
	manualset3
87002	4	398631	13	NULL	NULL	0	NULL	tumor promoters 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Homologs of the recently described mouse pro genes , that transfer sensitivity to promotion of neoplastic transformation by tumor promoters , have been cloned from a genomic library of the human nasopharyngeal carcinoma ( NPC ) cell line CNE2 .
	manualset3
87003	5	398631	13	NULL	NULL	NULL	NULL	genomic library	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Homologs of the recently described mouse pro genes , that transfer sensitivity to promotion of neoplastic transformation by tumor promoters , have been cloned from a genomic library of the human nasopharyngeal carcinoma ( NPC ) cell line CNE2 .
	manualset3
87004	6	398631	13	NULL	NULL	0	NULL	human nasopharyngeal carcinoma ( NPC ) cell line CNE2	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Homologs of the recently described mouse pro genes , that transfer sensitivity to promotion of neoplastic transformation by tumor promoters , have been cloned from a genomic library of the human nasopharyngeal carcinoma ( NPC ) cell line CNE2 .
	manualset3
87005	1	398632	13	NULL	NULL	0	NULL	Homology modeling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Homology modeling of human methylmalonyl-CoA mutase : a structural basis for point mutations causing methylmalonic aciduria .
	manualset3
87006	2	398632	13	NULL	NULL	0	NULL	human methylmalonyl-CoA mutase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Homology modeling of human methylmalonyl-CoA mutase : a structural basis for point mutations causing methylmalonic aciduria .
	manualset3
87007	3	398632	13	NULL	NULL	0	NULL	point mutations 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Homology modeling of human methylmalonyl-CoA mutase : a structural basis for point mutations causing methylmalonic aciduria .
	manualset3
87008	4	398632	13	NULL	NULL	0	NULL	methylmalonic aciduria	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Homology modeling of human methylmalonyl-CoA mutase : a structural basis for point mutations causing methylmalonic aciduria .
	manualset3
87009	1	398633	13	NULL	NULL	0	NULL	Homology models 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Homology models were constructed using the crystal structure of a bacterial homolog , the leucine transporter from Aquifex aeolicus , as the template and three slightly different sequence alignments .
	manualset3
87010	2	398633	13	NULL	NULL	NULL	NULL	crystal structure of a bacterial homolog	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Homology models were constructed using the crystal structure of a bacterial homolog , the leucine transporter from Aquifex aeolicus , as the template and three slightly different sequence alignments .
	manualset3
87011	3	398633	13	NULL	NULL	0	NULL	leucine transporter	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Homology models were constructed using the crystal structure of a bacterial homolog , the leucine transporter from Aquifex aeolicus , as the template and three slightly different sequence alignments .
	manualset3
87012	4	398633	13	NULL	NULL	0	NULL	 Aquifex aeolicus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Homology models were constructed using the crystal structure of a bacterial homolog , the leucine transporter from Aquifex aeolicus , as the template and three slightly different sequence alignments .
	manualset3
87013	5	398633	13	NULL	NULL	NULL	NULL	template 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Homology models were constructed using the crystal structure of a bacterial homolog , the leucine transporter from Aquifex aeolicus , as the template and three slightly different sequence alignments .
	manualset3
87014	6	398633	13	NULL	NULL	0	NULL	three 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Homology models were constructed using the crystal structure of a bacterial homolog , the leucine transporter from Aquifex aeolicus , as the template and three slightly different sequence alignments .
	manualset3
87015	7	398633	13	NULL	NULL	0	NULL	sequence alignments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Homology models were constructed using the crystal structure of a bacterial homolog , the leucine transporter from Aquifex aeolicus , as the template and three slightly different sequence alignments .
	manualset3
87016	1	398634	13	NULL	NULL	0	NULL	Hookworm anemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hookworm anemia , a deficiency disease .
	manualset3
87017	2	398634	13	NULL	NULL	0	NULL	deficiency disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hookworm anemia , a deficiency disease .
	manualset3
87018	1	398635	13	NULL	NULL	NULL	NULL	Hormonal changes	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hormonal changes during salinity-induced leaf senescence in tomato ( Solanum lycopersicum L. ) .
	manualset3
87019	2	398635	13	NULL	NULL	0	NULL	salinity-induced leaf senescence 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hormonal changes during salinity-induced leaf senescence in tomato ( Solanum lycopersicum L. ) .
	manualset3
87020	3	398635	13	NULL	NULL	0	NULL	tomato ( Solanum lycopersicum L. ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hormonal changes during salinity-induced leaf senescence in tomato ( Solanum lycopersicum L. ) .
	manualset3
87021	1	398636	13	NULL	NULL	0	NULL	The active metabolite of leflunomide A771726	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( The active metabolite of leflunomide A771726 inhibits proliferation and collagen synthesis of hepatic stellate cell ) .
	manualset3
87022	2	398636	13	NULL	NULL	0	NULL	proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( The active metabolite of leflunomide A771726 inhibits proliferation and collagen synthesis of hepatic stellate cell ) .
	manualset3
87023	3	398636	13	NULL	NULL	0	NULL	 collagen synthesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( The active metabolite of leflunomide A771726 inhibits proliferation and collagen synthesis of hepatic stellate cell ) .
	manualset3
87024	4	398636	13	NULL	NULL	0	NULL	hepatic stellate cell 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	( The active metabolite of leflunomide A771726 inhibits proliferation and collagen synthesis of hepatic stellate cell ) .
	manualset3
87025	1	398637	13	NULL	NULL	NULL	NULL	Hormonal factors	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hormonal factors may have a permissive role in thrombus formation or neoplastic vascular invasion .
	manualset3
87026	2	398637	13	NULL	NULL	NULL	NULL	thrombus formation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hormonal factors may have a permissive role in thrombus formation or neoplastic vascular invasion .
	manualset3
87027	3	398637	13	NULL	NULL	0	NULL	 neoplastic vascular invasion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hormonal factors may have a permissive role in thrombus formation or neoplastic vascular invasion .
	manualset3
87028	1	398638	13	NULL	NULL	NULL	NULL	Hormonal stimulation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hormonal stimulation of ribosomal RNA synthesis in Achlya ambisexualis .
	manualset3
87029	2	398638	13	NULL	NULL	0	NULL	ribosomal RNA synthesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hormonal stimulation of ribosomal RNA synthesis in Achlya ambisexualis .
	manualset3
87030	3	398638	13	NULL	NULL	0	NULL	Achlya ambisexualis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hormonal stimulation of ribosomal RNA synthesis in Achlya ambisexualis .
	manualset3
87031	1	398639	13	NULL	NULL	0	NULL	Hormone replacement therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hormone replacement therapy to develop secondary sexual characteristics has been used for years whereas several growth promoting agents undergo clinical trials at the moment .
	manualset3
87032	2	398639	13	NULL	NULL	0	NULL	develop secondary sexual characteristics	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hormone replacement therapy to develop secondary sexual characteristics has been used for years whereas several growth promoting agents undergo clinical trials at the moment .
	manualset3
87033	3	398639	13	NULL	NULL	0	NULL	years	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Hormone replacement therapy to develop secondary sexual characteristics has been used for years whereas several growth promoting agents undergo clinical trials at the moment .
	manualset3
87034	4	398639	13	NULL	NULL	0	NULL	several growth promoting agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hormone replacement therapy to develop secondary sexual characteristics has been used for years whereas several growth promoting agents undergo clinical trials at the moment .
	manualset3
87035	5	398639	13	NULL	NULL	0	NULL	clinical trials 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hormone replacement therapy to develop secondary sexual characteristics has been used for years whereas several growth promoting agents undergo clinical trials at the moment .
	manualset3
87036	1	398640	13	NULL	NULL	0	NULL	Hormone therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hormone therapy of such cancer has so far been only mildly active , probably because we do not understand the role and mechanism of action of FSH and FSHR in the hypothalamo-pituitary-ovarian axis in development of such cancer .
	manualset3
87037	2	398640	13	NULL	NULL	0	NULL	cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hormone therapy of such cancer has so far been only mildly active , probably because we do not understand the role and mechanism of action of FSH and FSHR in the hypothalamo-pituitary-ovarian axis in development of such cancer .
	manualset3
87038	3	398640	13	NULL	NULL	0	NULL	mechanism of action of FSH 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hormone therapy of such cancer has so far been only mildly active , probably because we do not understand the role and mechanism of action of FSH and FSHR in the hypothalamo-pituitary-ovarian axis in development of such cancer .
	manualset3
87039	4	398640	13	NULL	NULL	0	NULL	mechanism of action of FSHR	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hormone therapy of such cancer has so far been only mildly active , probably because we do not understand the role and mechanism of action of FSH and FSHR in the hypothalamo-pituitary-ovarian axis in development of such cancer .
	manualset3
87040	5	398640	13	NULL	NULL	0	NULL	hypothalamo-pituitary-ovarian axis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Hormone therapy of such cancer has so far been only mildly active , probably because we do not understand the role and mechanism of action of FSH and FSHR in the hypothalamo-pituitary-ovarian axis in development of such cancer .
	manualset3
87041	6	398640	13	NULL	NULL	0	NULL	development of such cancer 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hormone therapy of such cancer has so far been only mildly active , probably because we do not understand the role and mechanism of action of FSH and FSHR in the hypothalamo-pituitary-ovarian axis in development of such cancer .
	manualset3
87042	1	398641	13	NULL	NULL	0	NULL	Hospital admission blood pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hospital admission blood pressure : a predictor for hypertension following endotracheal intubation .
	manualset3
87043	2	398641	13	NULL	NULL	0	NULL	hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hospital admission blood pressure : a predictor for hypertension following endotracheal intubation .
	manualset3
87044	3	398641	13	NULL	NULL	0	NULL	endotracheal intubation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hospital admission blood pressure : a predictor for hypertension following endotracheal intubation .
	manualset3
87045	1	398642	13	NULL	NULL	0	NULL	Hospital trust director	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Hospital trust director is cleared of dishonesty in case of misdiagnosed diabetes .
	manualset3
87046	2	398642	13	NULL	NULL	0	NULL	dishonesty	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hospital trust director is cleared of dishonesty in case of misdiagnosed diabetes .
	manualset3
87047	3	398642	13	NULL	NULL	0	NULL	 diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hospital trust director is cleared of dishonesty in case of misdiagnosed diabetes .
	manualset3
87048	1	398643	13	NULL	NULL	0	NULL	Hospitalization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hospitalization of the mother as a necessary measure for the prevention of physical and psycho-affective disorders in the hospitalized child ) .
	manualset3
87049	2	398643	13	NULL	NULL	NULL	NULL	mother	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hospitalization of the mother as a necessary measure for the prevention of physical and psycho-affective disorders in the hospitalized child ) .
	manualset3
87050	3	398643	13	NULL	NULL	NULL	NULL	prevention 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hospitalization of the mother as a necessary measure for the prevention of physical and psycho-affective disorders in the hospitalized child ) .
	manualset3
87051	4	398643	13	NULL	NULL	0	NULL	hospitalized child 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Hospitalization of the mother as a necessary measure for the prevention of physical and psycho-affective disorders in the hospitalized child ) .
	manualset3
87052	5	398643	13	NULL	NULL	0	NULL	physical and psycho-affective disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hospitalization of the mother as a necessary measure for the prevention of physical and psycho-affective disorders in the hospitalized child ) .
	manualset3
87053	1	398644	13	NULL	NULL	0	NULL	lipid peroxidation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( The activity of the lipid peroxidation processes in the mucosa of the rat small intestine and its morphofunctional state under acute irradiation and the administration of combined preparations created on a base of highly dispersed silica ) .
	manualset3
87054	2	398644	13	NULL	NULL	0	NULL	mucosa of the rat small intestine 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	( The activity of the lipid peroxidation processes in the mucosa of the rat small intestine and its morphofunctional state under acute irradiation and the administration of combined preparations created on a base of highly dispersed silica ) .
	manualset3
87055	3	398644	13	NULL	NULL	NULL	NULL	acute irradiation	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The activity of the lipid peroxidation processes in the mucosa of the rat small intestine and its morphofunctional state under acute irradiation and the administration of combined preparations created on a base of highly dispersed silica ) .
	manualset3
87056	4	398644	13	NULL	NULL	NULL	NULL	administration of combined preparations	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The activity of the lipid peroxidation processes in the mucosa of the rat small intestine and its morphofunctional state under acute irradiation and the administration of combined preparations created on a base of highly dispersed silica ) .
	manualset3
87057	5	398644	13	NULL	NULL	0	NULL	silica	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( The activity of the lipid peroxidation processes in the mucosa of the rat small intestine and its morphofunctional state under acute irradiation and the administration of combined preparations created on a base of highly dispersed silica ) .
	manualset3
87058	1	398645	13	NULL	NULL	0	NULL	Host-derived adiponectin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Host-derived adiponectin is tumor-suppressive and a novel therapeutic target for multiple myeloma and the associated bone disease .
	manualset3
87059	2	398645	13	NULL	NULL	0	NULL	tumor-suppressive 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Host-derived adiponectin is tumor-suppressive and a novel therapeutic target for multiple myeloma and the associated bone disease .
	manualset3
87060	3	398645	13	NULL	NULL	0	NULL	novel therapeutic target	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Host-derived adiponectin is tumor-suppressive and a novel therapeutic target for multiple myeloma and the associated bone disease .
	manualset3
87061	4	398645	13	NULL	NULL	0	NULL	multiple myeloma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Host-derived adiponectin is tumor-suppressive and a novel therapeutic target for multiple myeloma and the associated bone disease .
	manualset3
87062	5	398645	13	NULL	NULL	0	NULL	bone disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Host-derived adiponectin is tumor-suppressive and a novel therapeutic target for multiple myeloma and the associated bone disease .
	manualset3
87063	1	398646	13	NULL	NULL	0	NULL	Host defense pathways 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Host defense pathways against fungi : the basis for vaccines and immunotherapy .
	manualset3
87064	2	398646	13	NULL	NULL	0	NULL	fungi	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Host defense pathways against fungi : the basis for vaccines and immunotherapy .
	manualset3
87065	3	398646	13	NULL	NULL	NULL	NULL	vaccines	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Host defense pathways against fungi : the basis for vaccines and immunotherapy .
	manualset3
87066	4	398646	13	NULL	NULL	0	NULL	immunotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Host defense pathways against fungi : the basis for vaccines and immunotherapy .
	manualset3
87067	1	398647	13	NULL	NULL	0	NULL	Host populations	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Host populations , transmission efficiency , and therefore pathogen amplification vary spatially , thereby creating a heterogeneous surface that may be defined by remote sensing and statistical tools .
	manualset3
87068	2	398647	13	NULL	NULL	0	NULL	transmission efficiency	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Host populations , transmission efficiency , and therefore pathogen amplification vary spatially , thereby creating a heterogeneous surface that may be defined by remote sensing and statistical tools .
	manualset3
87069	3	398647	13	NULL	NULL	NULL	NULL	pathogen 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Host populations , transmission efficiency , and therefore pathogen amplification vary spatially , thereby creating a heterogeneous surface that may be defined by remote sensing and statistical tools .
	manualset3
87070	4	398647	13	NULL	NULL	0	NULL	amplification 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Host populations , transmission efficiency , and therefore pathogen amplification vary spatially , thereby creating a heterogeneous surface that may be defined by remote sensing and statistical tools .
	manualset3
87071	5	398647	13	NULL	NULL	0	NULL	 heterogeneous surface	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Host populations , transmission efficiency , and therefore pathogen amplification vary spatially , thereby creating a heterogeneous surface that may be defined by remote sensing and statistical tools .
	manualset3
87072	6	398647	13	NULL	NULL	0	NULL	remote sensing 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Host populations , transmission efficiency , and therefore pathogen amplification vary spatially , thereby creating a heterogeneous surface that may be defined by remote sensing and statistical tools .
	manualset3
87073	7	398647	13	NULL	NULL	0	NULL	statistical tools	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Host populations , transmission efficiency , and therefore pathogen amplification vary spatially , thereby creating a heterogeneous surface that may be defined by remote sensing and statistical tools .
	manualset3
87074	1	398648	13	NULL	NULL	0	NULL	Host 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Host resistance against Candida alibcans infection in mice with adjuvant induced arthritis .
	manualset3
87075	2	398648	13	NULL	NULL	0	NULL	 resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Host resistance against Candida alibcans infection in mice with adjuvant induced arthritis .
	manualset3
87076	3	398648	13	NULL	NULL	0	NULL	Candida alibcans infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Host resistance against Candida alibcans infection in mice with adjuvant induced arthritis .
	manualset3
87077	4	398648	13	NULL	NULL	0	NULL	mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Host resistance against Candida alibcans infection in mice with adjuvant induced arthritis .
	manualset3
87078	5	398648	13	NULL	NULL	0	NULL	adjuvant induced arthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Host resistance against Candida alibcans infection in mice with adjuvant induced arthritis .
	manualset3
87079	1	398649	13	NULL	NULL	0	NULL	Hotspots	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Hotspots of intraspecific diversity have been observed in most species , often within areas of putative Pleistocene refugia .
	manualset3
87080	2	398649	13	NULL	NULL	0	NULL	intraspecific diversity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hotspots of intraspecific diversity have been observed in most species , often within areas of putative Pleistocene refugia .
	manualset3
87081	3	398649	13	NULL	NULL	0	NULL	species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hotspots of intraspecific diversity have been observed in most species , often within areas of putative Pleistocene refugia .
	manualset3
87082	4	398649	13	NULL	NULL	NULL	NULL	areas of putative Pleistocene refugia 	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hotspots of intraspecific diversity have been observed in most species , often within areas of putative Pleistocene refugia .
	manualset3
87083	1	398650	13	NULL	NULL	0	NULL	Household products	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Household products containing acids , alkalies or detergents : toxic effects and their treatment .
	manualset3
87084	2	398650	13	NULL	NULL	0	NULL	acids 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Household products containing acids , alkalies or detergents : toxic effects and their treatment .
	manualset3
87085	3	398650	13	NULL	NULL	0	NULL	alkalies	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Household products containing acids , alkalies or detergents : toxic effects and their treatment .
	manualset3
87086	4	398650	13	NULL	NULL	0	NULL	detergents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Household products containing acids , alkalies or detergents : toxic effects and their treatment .
	manualset3
87087	5	398650	13	NULL	NULL	0	NULL	 toxic effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Household products containing acids , alkalies or detergents : toxic effects and their treatment .
	manualset3
87088	6	398650	13	NULL	NULL	0	NULL	 treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Household products containing acids , alkalies or detergents : toxic effects and their treatment .
	manualset3
87089	1	398651	13	NULL	NULL	0	NULL	 poise	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	How to keep your poise under pressure .
	manualset3
87179	2	398651	13	NULL	NULL	0	NULL	 pressure	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	How to keep your poise under pressure .
	manualset3
87090	1	398652	13	NULL	NULL	0	NULL	 anti-anginous	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( The anti-anginous action of FT-9 ) .
	manualset3
87091	2	398652	13	NULL	NULL	0	NULL	FT-9 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( The anti-anginous action of FT-9 ) .
	manualset3
87092	1	398653	13	NULL	NULL	0	NULL	ZAP 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	How ZAP recognizes its target RNA has been unclear .
	manualset3
87093	2	398653	13	NULL	NULL	0	NULL	RNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	How ZAP recognizes its target RNA has been unclear .
	manualset3
87094	1	398654	13	NULL	NULL	0	NULL	midwife	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	How a midwife can change attitudes .
	manualset3
87095	2	398654	13	NULL	NULL	0	NULL	attitudes	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	How a midwife can change attitudes .
	manualset3
87096	1	398655	13	NULL	NULL	0	NULL	aerobic glycolysis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	How aerobic glycolysis and apoptosis resistance are linked remains to be elucidated .
	manualset3
87097	2	398655	13	NULL	NULL	0	NULL	apoptosis resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	How aerobic glycolysis and apoptosis resistance are linked remains to be elucidated .
	manualset3
87098	1	398656	13	NULL	NULL	NULL	NULL	organs	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	How are the regular patterns of organs established along a plant stem and howare the transitions between different patterns regulated ?
	manualset3
87099	2	398656	13	NULL	NULL	NULL	NULL	plant stem	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	How are the regular patterns of organs established along a plant stem and howare the transitions between different patterns regulated ?
	manualset3
87101	3	398656	13	NULL	NULL	NULL	NULL	transitions 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	How are the regular patterns of organs established along a plant stem and howare the transitions between different patterns regulated ?
	manualset3
87102	1	398657	13	NULL	NULL	0	NULL	roots 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	How do roots manage to simultaneously communicate with neighboring plants , and with symbiotic and pathogenic organisms within this crowded rhizosphere ?
	manualset3
87104	2	398657	13	NULL	NULL	0	NULL	neighboring plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	How do roots manage to simultaneously communicate with neighboring plants , and with symbiotic and pathogenic organisms within this crowded rhizosphere ?
	manualset3
87106	3	398657	13	NULL	NULL	0	NULL	symbiotic organisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	How do roots manage to simultaneously communicate with neighboring plants , and with symbiotic and pathogenic organisms within this crowded rhizosphere ?
	manualset3
87108	4	398657	13	NULL	NULL	0	NULL	pathogenic organisms 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	How do roots manage to simultaneously communicate with neighboring plants , and with symbiotic and pathogenic organisms within this crowded rhizosphere ?
	manualset3
87114	5	398657	13	NULL	NULL	0	NULL	rhizosphere	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	How do roots manage to simultaneously communicate with neighboring plants , and with symbiotic and pathogenic organisms within this crowded rhizosphere ?
	manualset3
87118	1	398658	13	NULL	NULL	0	NULL	data	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	How do we collect data for surveillance of wound infection ?
	manualset3
87119	2	398658	13	NULL	NULL	NULL	NULL	surveillance	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	How do we collect data for surveillance of wound infection ?
	manualset3
87120	3	398658	13	NULL	NULL	0	NULL	wound infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	How do we collect data for surveillance of wound infection ?
	manualset3
87124	1	398659	13	NULL	NULL	0	NULL	ammonium	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	How does ammonium dynamically interact with benzene in aqueous media ?
	manualset3
87125	2	398659	13	NULL	NULL	0	NULL	benzene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	How does ammonium dynamically interact with benzene in aqueous media ?
	manualset3
87126	3	398659	13	NULL	NULL	0	NULL	aqueous media	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	How does ammonium dynamically interact with benzene in aqueous media ?
	manualset3
87131	1	398660	13	NULL	NULL	0	NULL	 photoreceptor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	How photoreceptor cells respond to light .
	manualset3
87132	2	398660	13	NULL	NULL	0	NULL	 light 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	How photoreceptor cells respond to light .
	manualset3
87183	1	398661	13	NULL	NULL	0	NULL	antialgesic action	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( The antialgesic action of hyaluronidase in the treatment of medicinal apical parodontitis after filling of the canal ) .
	manualset3
87184	2	398661	13	NULL	NULL	0	NULL	hyaluronidase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( The antialgesic action of hyaluronidase in the treatment of medicinal apical parodontitis after filling of the canal ) .
	manualset3
87187	3	398661	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( The antialgesic action of hyaluronidase in the treatment of medicinal apical parodontitis after filling of the canal ) .
	manualset3
87189	4	398661	13	NULL	NULL	0	NULL	medicinal apical parodontitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( The antialgesic action of hyaluronidase in the treatment of medicinal apical parodontitis after filling of the canal ) .
	manualset3
87190	5	398661	13	NULL	NULL	0	NULL	filling of the canal 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( The antialgesic action of hyaluronidase in the treatment of medicinal apical parodontitis after filling of the canal ) .
	manualset3
87194	1	398662	13	NULL	NULL	0	NULL	future doctors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	How prepared are our future doctors for HIV/AIDS ?
	manualset3
87195	2	398662	13	NULL	NULL	0	NULL	 HIV/AIDS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	How prepared are our future doctors for HIV/AIDS ?
	manualset3
87200	1	398663	13	NULL	NULL	0	NULL	H1N1 influenza	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	How the H1N1 influenza epidemic spread among university students in Japan : experience from Shinshu University .
	manualset3
87203	2	398663	13	NULL	NULL	0	NULL	 epidemic spread	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	How the H1N1 influenza epidemic spread among university students in Japan : experience from Shinshu University .
	manualset3
87204	3	398663	13	NULL	NULL	0	NULL	university students	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	How the H1N1 influenza epidemic spread among university students in Japan : experience from Shinshu University .
	manualset3
87205	4	398663	13	NULL	NULL	0	NULL	Japan	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	How the H1N1 influenza epidemic spread among university students in Japan : experience from Shinshu University .
	manualset3
87208	5	398663	13	NULL	NULL	0	NULL	Shinshu University	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	How the H1N1 influenza epidemic spread among university students in Japan : experience from Shinshu University .
	manualset3
87209	1	398664	13	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	How these cells maintain their identity , restricted localization , and fate is unknown and is fundamental to the control of BP and homeostasis of fluid and electrolytes .
	manualset3
87213	2	398664	13	NULL	NULL	0	NULL	localization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	How these cells maintain their identity , restricted localization , and fate is unknown and is fundamental to the control of BP and homeostasis of fluid and electrolytes .
	manualset3
87216	3	398664	13	NULL	NULL	NULL	NULL	BP	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	How these cells maintain their identity , restricted localization , and fate is unknown and is fundamental to the control of BP and homeostasis of fluid and electrolytes .
	manualset3
87217	4	398664	13	NULL	NULL	0	NULL	homeostasis of fluid 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	How these cells maintain their identity , restricted localization , and fate is unknown and is fundamental to the control of BP and homeostasis of fluid and electrolytes .
	manualset3
87219	5	398664	13	NULL	NULL	0	NULL	electrolytes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	How these cells maintain their identity , restricted localization , and fate is unknown and is fundamental to the control of BP and homeostasis of fluid and electrolytes .
	manualset3
87221	1	398665	13	NULL	NULL	0	NULL	ACA 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	How these changes and the multiple other provisions of the ACA will affect young adults during the next decade is uncertain , but it has the potential to lead to earlier diagnosis of cancer , less invasive cancer therapy , better quality of survival , and higher cure rates .
	manualset3
87223	2	398665	13	NULL	NULL	0	NULL	young adults	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	How these changes and the multiple other provisions of the ACA will affect young adults during the next decade is uncertain , but it has the potential to lead to earlier diagnosis of cancer , less invasive cancer therapy , better quality of survival , and higher cure rates .
	manualset3
87225	3	398665	13	NULL	NULL	0	NULL	decade 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	How these changes and the multiple other provisions of the ACA will affect young adults during the next decade is uncertain , but it has the potential to lead to earlier diagnosis of cancer , less invasive cancer therapy , better quality of survival , and higher cure rates .
	manualset3
87231	4	398665	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	How these changes and the multiple other provisions of the ACA will affect young adults during the next decade is uncertain , but it has the potential to lead to earlier diagnosis of cancer , less invasive cancer therapy , better quality of survival , and higher cure rates .
	manualset3
87233	5	398665	13	NULL	NULL	0	NULL	cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	How these changes and the multiple other provisions of the ACA will affect young adults during the next decade is uncertain , but it has the potential to lead to earlier diagnosis of cancer , less invasive cancer therapy , better quality of survival , and higher cure rates .
	manualset3
87234	6	398665	13	NULL	NULL	0	NULL	 less invasive cancer therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	How these changes and the multiple other provisions of the ACA will affect young adults during the next decade is uncertain , but it has the potential to lead to earlier diagnosis of cancer , less invasive cancer therapy , better quality of survival , and higher cure rates .
	manualset3
87236	7	398665	13	NULL	NULL	0	NULL	better quality of survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	How these changes and the multiple other provisions of the ACA will affect young adults during the next decade is uncertain , but it has the potential to lead to earlier diagnosis of cancer , less invasive cancer therapy , better quality of survival , and higher cure rates .
	manualset3
87237	8	398665	13	NULL	NULL	0	NULL	higher cure rates 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	How these changes and the multiple other provisions of the ACA will affect young adults during the next decade is uncertain , but it has the potential to lead to earlier diagnosis of cancer , less invasive cancer therapy , better quality of survival , and higher cure rates .
	manualset3
87262	1	398666	13	NULL	NULL	0	NULL	HCV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Howerver , even in cases of tight association , the mechanisms through which HCV may promote or induce extrahepatic manifestations remain unclear and merit further investigations .
	manualset3
87264	2	398666	13	NULL	NULL	0	NULL	mechanisms 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Howerver , even in cases of tight association , the mechanisms through which HCV may promote or induce extrahepatic manifestations remain unclear and merit further investigations .
	manualset3
87267	3	398666	13	NULL	NULL	0	NULL	extrahepatic manifestations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Howerver , even in cases of tight association , the mechanisms through which HCV may promote or induce extrahepatic manifestations remain unclear and merit further investigations .
	manualset3
87268	4	398666	13	NULL	NULL	0	NULL	 investigations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Howerver , even in cases of tight association , the mechanisms through which HCV may promote or induce extrahepatic manifestations remain unclear and merit further investigations .
	manualset3
87275	1	398667	13	NULL	NULL	0	NULL	 ( 125I ) iodoarylazidoprazosin photoaffinity labeling 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , ( 125I ) iodoarylazidoprazosin photoaffinity labeling of the chimeric Pgp and its binding competition with cyclosporin A , showed that cyclosporin A competed for the photoaffinity labeling .
	manualset3
87276	2	398667	13	NULL	NULL	0	NULL	chimeric Pgp	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , ( 125I ) iodoarylazidoprazosin photoaffinity labeling of the chimeric Pgp and its binding competition with cyclosporin A , showed that cyclosporin A competed for the photoaffinity labeling .
	manualset3
87277	3	398667	13	NULL	NULL	0	NULL	 binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , ( 125I ) iodoarylazidoprazosin photoaffinity labeling of the chimeric Pgp and its binding competition with cyclosporin A , showed that cyclosporin A competed for the photoaffinity labeling .
	manualset3
87278	4	398667	13	NULL	NULL	0	NULL	cyclosporin A	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , ( 125I ) iodoarylazidoprazosin photoaffinity labeling of the chimeric Pgp and its binding competition with cyclosporin A , showed that cyclosporin A competed for the photoaffinity labeling .
	manualset3
87279	5	398667	13	NULL	NULL	0	NULL	cyclosporin A	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , ( 125I ) iodoarylazidoprazosin photoaffinity labeling of the chimeric Pgp and its binding competition with cyclosporin A , showed that cyclosporin A competed for the photoaffinity labeling .
	manualset3
87280	6	398667	13	NULL	NULL	0	NULL	 photoaffinity labeling 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , ( 125I ) iodoarylazidoprazosin photoaffinity labeling of the chimeric Pgp and its binding competition with cyclosporin A , showed that cyclosporin A competed for the photoaffinity labeling .
	manualset3
87281	1	398668	13	NULL	NULL	0	NULL	pyrexia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , his pyrexia continued and he developed repeating visual and hearing impairment reacting to steroid .
	manualset3
87282	2	398668	13	NULL	NULL	0	NULL	visual and hearing impairment 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , his pyrexia continued and he developed repeating visual and hearing impairment reacting to steroid .
	manualset3
87283	3	398668	13	NULL	NULL	NULL	NULL	steroid	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , his pyrexia continued and he developed repeating visual and hearing impairment reacting to steroid .
	manualset3
87284	1	398669	13	NULL	NULL	0	NULL	AGEP	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , our case describes the rare presentation of AGEP induced by erlotinib .
	manualset3
87285	2	398669	13	NULL	NULL	0	NULL	erlotinib	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , our case describes the rare presentation of AGEP induced by erlotinib .
	manualset3
87286	1	398670	13	NULL	NULL	0	NULL	urban populations 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , our focus will be on some of the more vulnerable urban populations who are most profoundly affected by SDH .
	manualset3
87287	2	398670	13	NULL	NULL	NULL	NULL	 SDH 	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , our focus will be on some of the more vulnerable urban populations who are most profoundly affected by SDH .
	manualset3
87288	1	398671	13	NULL	NULL	NULL	NULL	 courtship regulation 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , their acute physiological roles in courtship regulation still largely remain unknown .
	manualset3
87289	1	398672	13	NULL	NULL	0	NULL	reproducibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , their reproducibility varied highly ( CV 9-40 % ) .
	manualset3
87290	2	398672	13	NULL	NULL	0	NULL	CV 9-40 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , their reproducibility varied highly ( CV 9-40 % ) .
	manualset3
87291	1	398673	13	NULL	NULL	0	NULL	1 month	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	However , 1 month after the chemotherapy , she developed ALL .
	manualset3
87292	2	398673	13	NULL	NULL	0	NULL	chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , 1 month after the chemotherapy , she developed ALL .
	manualset3
87293	3	398673	13	NULL	NULL	0	NULL	 ALL	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	However , 1 month after the chemotherapy , she developed ALL .
	manualset3
87294	1	398674	13	NULL	NULL	0	NULL	3 - ( methylthio ) catechol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , 3 - ( methylthio ) catechol is a very poor substrate for catechol 1 , 2-dioxygenase ( 0.8 % of the rate of catechol ) , but it is a potent competitive inhibitor ( Ki = 0.6 microM ) .
	manualset3
87295	2	398674	13	NULL	NULL	0	NULL	catechol 1 , 2-dioxygenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , 3 - ( methylthio ) catechol is a very poor substrate for catechol 1 , 2-dioxygenase ( 0.8 % of the rate of catechol ) , but it is a potent competitive inhibitor ( Ki = 0.6 microM ) .
	manualset3
87296	3	398674	13	NULL	NULL	0	NULL	0.8 % of the rate of catechol 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , 3 - ( methylthio ) catechol is a very poor substrate for catechol 1 , 2-dioxygenase ( 0.8 % of the rate of catechol ) , but it is a potent competitive inhibitor ( Ki = 0.6 microM ) .
	manualset3
87297	4	398674	13	NULL	NULL	0	NULL	inhibitor	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , 3 - ( methylthio ) catechol is a very poor substrate for catechol 1 , 2-dioxygenase ( 0.8 % of the rate of catechol ) , but it is a potent competitive inhibitor ( Ki = 0.6 microM ) .
	manualset3
87298	5	398674	13	NULL	NULL	0	NULL	Ki = 0.6 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , 3 - ( methylthio ) catechol is a very poor substrate for catechol 1 , 2-dioxygenase ( 0.8 % of the rate of catechol ) , but it is a potent competitive inhibitor ( Ki = 0.6 microM ) .
	manualset3
87299	1	398675	13	NULL	NULL	0	NULL	Analysis of properties of single molecules 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Analysis of properties of single molecules in vivo or ... why small fish is better than empty dish ) .
	manualset3
87300	2	398675	13	NULL	NULL	NULL	NULL	fish	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Analysis of properties of single molecules in vivo or ... why small fish is better than empty dish ) .
	manualset3
87301	3	398675	13	NULL	NULL	0	NULL	dish	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( Analysis of properties of single molecules in vivo or ... why small fish is better than empty dish ) .
	manualset3
87302	1	398676	13	NULL	NULL	0	NULL	cyclic AMP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	( The biological role of cyclic AMP ) .
	manualset3
87652	2	398676	13	NULL	NULL	0	NULL	biological role 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( The biological role of cyclic AMP ) .
	manualset3
87303	1	398677	13	NULL	NULL	0	NULL	8 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	However , 8 weeks after implantation the UBM-treated defect area showed significantly greater ( p & lt ; 0.05 ) regional systolic contraction compared to the myocardial defects repaired with by Dacron ( 3.3 + / - 1.3 % vs. -1.8 + / - 1.1 % ; respectively ) .
	manualset3
87304	2	398677	13	NULL	NULL	NULL	NULL	implantation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , 8 weeks after implantation the UBM-treated defect area showed significantly greater ( p & lt ; 0.05 ) regional systolic contraction compared to the myocardial defects repaired with by Dacron ( 3.3 + / - 1.3 % vs. -1.8 + / - 1.1 % ; respectively ) .
	manualset3
87305	3	398677	13	NULL	NULL	0	NULL	UBM-treated defect area 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , 8 weeks after implantation the UBM-treated defect area showed significantly greater ( p & lt ; 0.05 ) regional systolic contraction compared to the myocardial defects repaired with by Dacron ( 3.3 + / - 1.3 % vs. -1.8 + / - 1.1 % ; respectively ) .
	manualset3
87306	4	398677	13	NULL	NULL	0	NULL	p & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , 8 weeks after implantation the UBM-treated defect area showed significantly greater ( p & lt ; 0.05 ) regional systolic contraction compared to the myocardial defects repaired with by Dacron ( 3.3 + / - 1.3 % vs. -1.8 + / - 1.1 % ; respectively ) .
	manualset3
87307	5	398677	13	NULL	NULL	0	NULL	regional systolic contraction 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , 8 weeks after implantation the UBM-treated defect area showed significantly greater ( p & lt ; 0.05 ) regional systolic contraction compared to the myocardial defects repaired with by Dacron ( 3.3 + / - 1.3 % vs. -1.8 + / - 1.1 % ; respectively ) .
	manualset3
87308	6	398677	13	NULL	NULL	0	NULL	myocardial defects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , 8 weeks after implantation the UBM-treated defect area showed significantly greater ( p & lt ; 0.05 ) regional systolic contraction compared to the myocardial defects repaired with by Dacron ( 3.3 + / - 1.3 % vs. -1.8 + / - 1.1 % ; respectively ) .
	manualset3
87309	7	398677	13	NULL	NULL	0	NULL	Dacron	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	However , 8 weeks after implantation the UBM-treated defect area showed significantly greater ( p & lt ; 0.05 ) regional systolic contraction compared to the myocardial defects repaired with by Dacron ( 3.3 + / - 1.3 % vs. -1.8 + / - 1.1 % ; respectively ) .
	manualset3
87310	8	398677	13	NULL	NULL	0	NULL	3.3 + / - 1.3 % vs. -1.8 + / - 1.1 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , 8 weeks after implantation the UBM-treated defect area showed significantly greater ( p & lt ; 0.05 ) regional systolic contraction compared to the myocardial defects repaired with by Dacron ( 3.3 + / - 1.3 % vs. -1.8 + / - 1.1 % ; respectively ) .
	manualset3
87311	1	398678	13	NULL	NULL	0	NULL	ALA pentyl ester	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , ALA pentyl ester slightly increased the in vivo PpIX fluorescence in early ( pre ) malignant lesions in hairless mouse skin compared to ALA. .
	manualset3
87312	2	398678	13	NULL	NULL	NULL	NULL	 PpIX fluorescence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , ALA pentyl ester slightly increased the in vivo PpIX fluorescence in early ( pre ) malignant lesions in hairless mouse skin compared to ALA. .
	manualset3
87313	3	398678	13	NULL	NULL	NULL	NULL	early ( pre ) malignant lesions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , ALA pentyl ester slightly increased the in vivo PpIX fluorescence in early ( pre ) malignant lesions in hairless mouse skin compared to ALA. .
	manualset3
87314	4	398678	13	NULL	NULL	0	NULL	hairless mouse skin 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	However , ALA pentyl ester slightly increased the in vivo PpIX fluorescence in early ( pre ) malignant lesions in hairless mouse skin compared to ALA. .
	manualset3
87315	5	398678	13	NULL	NULL	0	NULL	ALA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , ALA pentyl ester slightly increased the in vivo PpIX fluorescence in early ( pre ) malignant lesions in hairless mouse skin compared to ALA. .
	manualset3
87316	1	398679	13	NULL	NULL	0	NULL	AMG517 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , AMG517 , a TRPV1 antagonist , presents several clinical limitations that include the induction of severe hyperthermia .
	manualset3
87317	2	398679	13	NULL	NULL	0	NULL	TRPV1 antagonist	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , AMG517 , a TRPV1 antagonist , presents several clinical limitations that include the induction of severe hyperthermia .
	manualset3
87318	3	398679	13	NULL	NULL	0	NULL	clinical limitations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , AMG517 , a TRPV1 antagonist , presents several clinical limitations that include the induction of severe hyperthermia .
	manualset3
87319	4	398679	13	NULL	NULL	0	NULL	severe hyperthermia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , AMG517 , a TRPV1 antagonist , presents several clinical limitations that include the induction of severe hyperthermia .
	manualset3
87320	1	398680	13	NULL	NULL	0	NULL	AngII 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , AngII did increase O2 * - when the tissue strips were preincubated with the NO scavenger 2 - ( 4-carboxyphenyl ) -4 , 4 , 5 , 5 - tetramethylimidazoline-1-oxyl-3-oxide ( carboxy-PTIO ) , indicating that cross-talk of O2 * - from mTAL to the VR occurred but was normally inhibited by NO. .
	manualset3
87321	2	398680	13	NULL	NULL	0	NULL	O2 *	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	However , AngII did increase O2 * - when the tissue strips were preincubated with the NO scavenger 2 - ( 4-carboxyphenyl ) -4 , 4 , 5 , 5 - tetramethylimidazoline-1-oxyl-3-oxide ( carboxy-PTIO ) , indicating that cross-talk of O2 * - from mTAL to the VR occurred but was normally inhibited by NO. .
	manualset3
87322	3	398680	13	NULL	NULL	NULL	NULL	tissue	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , AngII did increase O2 * - when the tissue strips were preincubated with the NO scavenger 2 - ( 4-carboxyphenyl ) -4 , 4 , 5 , 5 - tetramethylimidazoline-1-oxyl-3-oxide ( carboxy-PTIO ) , indicating that cross-talk of O2 * - from mTAL to the VR occurred but was normally inhibited by NO. .
	manualset3
87323	4	398680	13	NULL	NULL	NULL	NULL	NO scavenger	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , AngII did increase O2 * - when the tissue strips were preincubated with the NO scavenger 2 - ( 4-carboxyphenyl ) -4 , 4 , 5 , 5 - tetramethylimidazoline-1-oxyl-3-oxide ( carboxy-PTIO ) , indicating that cross-talk of O2 * - from mTAL to the VR occurred but was normally inhibited by NO. .
	manualset3
87326	5	398680	13	NULL	NULL	0	NULL	2 - ( 4-carboxyphenyl ) -4 , 4 , 5 , 5 - tetramethylimidazoline-1-oxyl-3-oxide ( carboxy-PTIO )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , AngII did increase O2 * - when the tissue strips were preincubated with the NO scavenger 2 - ( 4-carboxyphenyl ) -4 , 4 , 5 , 5 - tetramethylimidazoline-1-oxyl-3-oxide ( carboxy-PTIO ) , indicating that cross-talk of O2 * - from mTAL to the VR occurred but was normally inhibited by NO. .
	manualset3
87327	6	398680	13	NULL	NULL	NULL	NULL	cross-talk of O2 *	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , AngII did increase O2 * - when the tissue strips were preincubated with the NO scavenger 2 - ( 4-carboxyphenyl ) -4 , 4 , 5 , 5 - tetramethylimidazoline-1-oxyl-3-oxide ( carboxy-PTIO ) , indicating that cross-talk of O2 * - from mTAL to the VR occurred but was normally inhibited by NO. .
	manualset3
87328	7	398680	13	NULL	NULL	0	NULL	mTAL	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , AngII did increase O2 * - when the tissue strips were preincubated with the NO scavenger 2 - ( 4-carboxyphenyl ) -4 , 4 , 5 , 5 - tetramethylimidazoline-1-oxyl-3-oxide ( carboxy-PTIO ) , indicating that cross-talk of O2 * - from mTAL to the VR occurred but was normally inhibited by NO. .
	manualset3
87329	8	398680	13	NULL	NULL	0	NULL	VR	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , AngII did increase O2 * - when the tissue strips were preincubated with the NO scavenger 2 - ( 4-carboxyphenyl ) -4 , 4 , 5 , 5 - tetramethylimidazoline-1-oxyl-3-oxide ( carboxy-PTIO ) , indicating that cross-talk of O2 * - from mTAL to the VR occurred but was normally inhibited by NO. .
	manualset3
87330	9	398680	13	NULL	NULL	0	NULL	NO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , AngII did increase O2 * - when the tissue strips were preincubated with the NO scavenger 2 - ( 4-carboxyphenyl ) -4 , 4 , 5 , 5 - tetramethylimidazoline-1-oxyl-3-oxide ( carboxy-PTIO ) , indicating that cross-talk of O2 * - from mTAL to the VR occurred but was normally inhibited by NO. .
	manualset3
87331	1	398681	13	NULL	NULL	0	NULL	Arabidopsis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , Arabidopsis showed a higher number of significantly altered mass features than Thellungiella .
	manualset3
87332	2	398681	13	NULL	NULL	0	NULL	Thellungiella 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , Arabidopsis showed a higher number of significantly altered mass features than Thellungiella .
	manualset3
87333	3	398681	13	NULL	NULL	NULL	NULL	features 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , Arabidopsis showed a higher number of significantly altered mass features than Thellungiella .
	manualset3
87653	4	398681	13	NULL	NULL	0	NULL	higher number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , Arabidopsis showed a higher number of significantly altered mass features than Thellungiella .
	manualset3
87334	1	398682	13	NULL	NULL	0	NULL	Au nanoparticles	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , Au nanoparticles undergo charge equilibration with TiO ( 2 ) nanoparticles and shift the apparent Fermi level of the composite to more negative potentials .
	manualset3
87335	2	398682	13	NULL	NULL	NULL	NULL	charge equilibration	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , Au nanoparticles undergo charge equilibration with TiO ( 2 ) nanoparticles and shift the apparent Fermi level of the composite to more negative potentials .
	manualset3
87336	3	398682	13	NULL	NULL	0	NULL	TiO ( 2 ) nanoparticles	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , Au nanoparticles undergo charge equilibration with TiO ( 2 ) nanoparticles and shift the apparent Fermi level of the composite to more negative potentials .
	manualset3
87654	4	398682	13	NULL	NULL	0	NULL	apparent Fermi level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , Au nanoparticles undergo charge equilibration with TiO ( 2 ) nanoparticles and shift the apparent Fermi level of the composite to more negative potentials .
	manualset3
87655	5	398682	13	NULL	NULL	0	NULL	negative potentials	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , Au nanoparticles undergo charge equilibration with TiO ( 2 ) nanoparticles and shift the apparent Fermi level of the composite to more negative potentials .
	manualset3
87337	1	398683	13	NULL	NULL	0	NULL	BAPTA-AM	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , BAPTA-AM did not interfere with the ER-stress response pathway that triggers the expression of GRP 78 .
	manualset3
87338	2	398683	13	NULL	NULL	0	NULL	ER-stress response pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , BAPTA-AM did not interfere with the ER-stress response pathway that triggers the expression of GRP 78 .
	manualset3
87339	3	398683	13	NULL	NULL	0	NULL	expression of GRP 78	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , BAPTA-AM did not interfere with the ER-stress response pathway that triggers the expression of GRP 78 .
	manualset3
87340	1	398684	13	NULL	NULL	0	NULL	GABAergic afferents 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , GABAergic afferents account for only a fraction of A15 synaptic input and do not appear to vary with season .
	manualset3
87341	2	398684	13	NULL	NULL	0	NULL	A15 synaptic input	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , GABAergic afferents account for only a fraction of A15 synaptic input and do not appear to vary with season .
	manualset3
87342	3	398684	13	NULL	NULL	0	NULL	season	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , GABAergic afferents account for only a fraction of A15 synaptic input and do not appear to vary with season .
	manualset3
87343	1	398685	13	NULL	NULL	0	NULL	 IK	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , IK has a nonlinear dependence on ( V-EK ) well described by the Goldman-Hodgkin-Katz equation that determines the voltage dependence of gK .
	manualset3
87344	2	398685	13	NULL	NULL	0	NULL	V-EK	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , IK has a nonlinear dependence on ( V-EK ) well described by the Goldman-Hodgkin-Katz equation that determines the voltage dependence of gK .
	manualset3
87345	3	398685	13	NULL	NULL	0	NULL	Goldman-Hodgkin-Katz equation 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	However , IK has a nonlinear dependence on ( V-EK ) well described by the Goldman-Hodgkin-Katz equation that determines the voltage dependence of gK .
	manualset3
87346	4	398685	13	NULL	NULL	NULL	NULL	voltage dependence	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , IK has a nonlinear dependence on ( V-EK ) well described by the Goldman-Hodgkin-Katz equation that determines the voltage dependence of gK .
	manualset3
87347	5	398685	13	NULL	NULL	0	NULL	 gK 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , IK has a nonlinear dependence on ( V-EK ) well described by the Goldman-Hodgkin-Katz equation that determines the voltage dependence of gK .
	manualset3
87656	6	398685	13	NULL	NULL	0	NULL	 nonlinear dependence 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , IK has a nonlinear dependence on ( V-EK ) well described by the Goldman-Hodgkin-Katz equation that determines the voltage dependence of gK .
	manualset3
87348	1	398686	13	NULL	NULL	0	NULL	IgE antibodies	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , IgE antibodies to a serum dilution of 1 : 200 specific for several components of the leaf extract were seen in serum from the dog that had anaphylactic shock after exposure to sap .
	manualset3
87349	2	398686	13	NULL	NULL	NULL	NULL	serum dilution of 1 : 200	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , IgE antibodies to a serum dilution of 1 : 200 specific for several components of the leaf extract were seen in serum from the dog that had anaphylactic shock after exposure to sap .
	manualset3
87350	3	398686	13	NULL	NULL	NULL	NULL	components of the leaf extract 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , IgE antibodies to a serum dilution of 1 : 200 specific for several components of the leaf extract were seen in serum from the dog that had anaphylactic shock after exposure to sap .
	manualset3
87351	4	398686	13	NULL	NULL	NULL	NULL	serum 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , IgE antibodies to a serum dilution of 1 : 200 specific for several components of the leaf extract were seen in serum from the dog that had anaphylactic shock after exposure to sap .
	manualset3
87352	5	398686	13	NULL	NULL	0	NULL	dog	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , IgE antibodies to a serum dilution of 1 : 200 specific for several components of the leaf extract were seen in serum from the dog that had anaphylactic shock after exposure to sap .
	manualset3
87353	6	398686	13	NULL	NULL	0	NULL	anaphylactic shock	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , IgE antibodies to a serum dilution of 1 : 200 specific for several components of the leaf extract were seen in serum from the dog that had anaphylactic shock after exposure to sap .
	manualset3
87354	7	398686	13	NULL	NULL	0	NULL	sap 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , IgE antibodies to a serum dilution of 1 : 200 specific for several components of the leaf extract were seen in serum from the dog that had anaphylactic shock after exposure to sap .
	manualset3
87355	1	398687	13	NULL	NULL	0	NULL	Japanese patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , Japanese patients undergoing dialysis might be less tolerant of sevelamer treatment , and it is likely to cause hypocalcemia because their dietary Ca intake is less than that in European and American patients .
	manualset3
87356	2	398687	13	NULL	NULL	0	NULL	dialysis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , Japanese patients undergoing dialysis might be less tolerant of sevelamer treatment , and it is likely to cause hypocalcemia because their dietary Ca intake is less than that in European and American patients .
	manualset3
87357	3	398687	13	NULL	NULL	0	NULL	sevelamer treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , Japanese patients undergoing dialysis might be less tolerant of sevelamer treatment , and it is likely to cause hypocalcemia because their dietary Ca intake is less than that in European and American patients .
	manualset3
87358	4	398687	13	NULL	NULL	0	NULL	hypocalcemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , Japanese patients undergoing dialysis might be less tolerant of sevelamer treatment , and it is likely to cause hypocalcemia because their dietary Ca intake is less than that in European and American patients .
	manualset3
87359	5	398687	13	NULL	NULL	0	NULL	Ca intake	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	However , Japanese patients undergoing dialysis might be less tolerant of sevelamer treatment , and it is likely to cause hypocalcemia because their dietary Ca intake is less than that in European and American patients .
	manualset3
87360	6	398687	13	NULL	NULL	0	NULL	European patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , Japanese patients undergoing dialysis might be less tolerant of sevelamer treatment , and it is likely to cause hypocalcemia because their dietary Ca intake is less than that in European and American patients .
	manualset3
87361	7	398687	13	NULL	NULL	0	NULL	American patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , Japanese patients undergoing dialysis might be less tolerant of sevelamer treatment , and it is likely to cause hypocalcemia because their dietary Ca intake is less than that in European and American patients .
	manualset3
87362	1	398688	13	NULL	NULL	0	NULL	Mg2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	However , Mg2 + enhanced equally by a factor of 3 affinities of high - and low-affinity binding sites as evidenced by SMS 201.995 displacement curves without modifying the ratio between high and low affinity sites .
	manualset3
87363	2	398688	13	NULL	NULL	0	NULL	SMS 201.995 displacement curves	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	However , Mg2 + enhanced equally by a factor of 3 affinities of high - and low-affinity binding sites as evidenced by SMS 201.995 displacement curves without modifying the ratio between high and low affinity sites .
	manualset3
87659	3	398688	13	NULL	NULL	0	NULL	factor of 3 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , Mg2 + enhanced equally by a factor of 3 affinities of high - and low-affinity binding sites as evidenced by SMS 201.995 displacement curves without modifying the ratio between high and low affinity sites .
	manualset3
87660	4	398688	13	NULL	NULL	NULL	NULL	high - and low-affinity binding sites 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , Mg2 + enhanced equally by a factor of 3 affinities of high - and low-affinity binding sites as evidenced by SMS 201.995 displacement curves without modifying the ratio between high and low affinity sites .
	manualset3
87661	5	398688	13	NULL	NULL	0	NULL	ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , Mg2 + enhanced equally by a factor of 3 affinities of high - and low-affinity binding sites as evidenced by SMS 201.995 displacement curves without modifying the ratio between high and low affinity sites .
	manualset3
87662	6	398688	13	NULL	NULL	0	NULL	high and low affinity sites 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , Mg2 + enhanced equally by a factor of 3 affinities of high - and low-affinity binding sites as evidenced by SMS 201.995 displacement curves without modifying the ratio between high and low affinity sites .
	manualset3
87364	1	398689	13	NULL	NULL	0	NULL	North American signal crayfish Pacifastacus leniusculus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , North American signal crayfish Pacifastacus leniusculus were recently discovered in a water-course that has been repeatedly hit by the plague .
	manualset3
87365	2	398689	13	NULL	NULL	0	NULL	water-course	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , North American signal crayfish Pacifastacus leniusculus were recently discovered in a water-course that has been repeatedly hit by the plague .
	manualset3
87366	3	398689	13	NULL	NULL	0	NULL	plague	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	However , North American signal crayfish Pacifastacus leniusculus were recently discovered in a water-course that has been repeatedly hit by the plague .
	manualset3
87367	1	398690	13	NULL	NULL	0	NULL	PBP2a	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , PBP2a did not cross-link the peptide stems of glycan chains in vitro .
	manualset3
87368	2	398690	13	NULL	NULL	0	NULL	cross-link	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , PBP2a did not cross-link the peptide stems of glycan chains in vitro .
	manualset3
87369	3	398690	13	NULL	NULL	0	NULL	peptide stems of glycan chains	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	However , PBP2a did not cross-link the peptide stems of glycan chains in vitro .
	manualset3
87370	1	398691	13	NULL	NULL	0	NULL	PPCM	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	However , PPCM differs from autoimmune IDCM in that ( a ) it is associated with unique sets of autoantibodies and autoantigens , ( b ) it has a relatively rapid onset , and ( c ) it exclusively affects pregnant women .
	manualset3
87371	2	398691	13	NULL	NULL	0	NULL	autoimmune IDCM 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	However , PPCM differs from autoimmune IDCM in that ( a ) it is associated with unique sets of autoantibodies and autoantigens , ( b ) it has a relatively rapid onset , and ( c ) it exclusively affects pregnant women .
	manualset3
87372	3	398691	13	NULL	NULL	0	NULL	autoantibodies	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , PPCM differs from autoimmune IDCM in that ( a ) it is associated with unique sets of autoantibodies and autoantigens , ( b ) it has a relatively rapid onset , and ( c ) it exclusively affects pregnant women .
	manualset3
87373	4	398691	13	NULL	NULL	0	NULL	autoantigens	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , PPCM differs from autoimmune IDCM in that ( a ) it is associated with unique sets of autoantibodies and autoantigens , ( b ) it has a relatively rapid onset , and ( c ) it exclusively affects pregnant women .
	manualset3
87374	5	398691	13	NULL	NULL	0	NULL	rapid onset	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , PPCM differs from autoimmune IDCM in that ( a ) it is associated with unique sets of autoantibodies and autoantigens , ( b ) it has a relatively rapid onset , and ( c ) it exclusively affects pregnant women .
	manualset3
87375	6	398691	13	NULL	NULL	0	NULL	pregnant women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , PPCM differs from autoimmune IDCM in that ( a ) it is associated with unique sets of autoantibodies and autoantigens , ( b ) it has a relatively rapid onset , and ( c ) it exclusively affects pregnant women .
	manualset3
87376	1	398692	13	NULL	NULL	0	NULL	Thy-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , Thy-1 was never expressed until the total age of 10 weeks .
	manualset3
87377	2	398692	13	NULL	NULL	0	NULL	age of 10 weeks 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	However , Thy-1 was never expressed until the total age of 10 weeks .
	manualset3
87378	1	398693	13	NULL	NULL	0	NULL	Yamanouchi	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	However , Yamanouchi and Pfizer discontinued the co-development and marketing agreement for conivaptan .
	manualset3
87379	2	398693	13	NULL	NULL	0	NULL	Pfizer	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	However , Yamanouchi and Pfizer discontinued the co-development and marketing agreement for conivaptan .
	manualset3
87380	3	398693	13	NULL	NULL	0	NULL	marketing agreement	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , Yamanouchi and Pfizer discontinued the co-development and marketing agreement for conivaptan .
	manualset3
87381	4	398693	13	NULL	NULL	0	NULL	conivaptan	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , Yamanouchi and Pfizer discontinued the co-development and marketing agreement for conivaptan .
	manualset3
87382	1	398694	13	NULL	NULL	NULL	NULL	Nesselt number	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , a bulk Nesselt number should not be used to estimate heat loss from a live sheep in a hot environment if the windspeed is below about 4 m s-1 because the relation between mean surface temperature , Nusselt number and convective heat flux is not unique .
	manualset3
87383	2	398694	13	NULL	NULL	NULL	NULL	heat loss 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , a bulk Nesselt number should not be used to estimate heat loss from a live sheep in a hot environment if the windspeed is below about 4 m s-1 because the relation between mean surface temperature , Nusselt number and convective heat flux is not unique .
	manualset3
87384	3	398694	13	NULL	NULL	0	NULL	live sheep	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , a bulk Nesselt number should not be used to estimate heat loss from a live sheep in a hot environment if the windspeed is below about 4 m s-1 because the relation between mean surface temperature , Nusselt number and convective heat flux is not unique .
	manualset3
87385	4	398694	13	NULL	NULL	0	NULL	hot environment 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , a bulk Nesselt number should not be used to estimate heat loss from a live sheep in a hot environment if the windspeed is below about 4 m s-1 because the relation between mean surface temperature , Nusselt number and convective heat flux is not unique .
	manualset3
87386	5	398694	13	NULL	NULL	0	NULL	windspeed	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , a bulk Nesselt number should not be used to estimate heat loss from a live sheep in a hot environment if the windspeed is below about 4 m s-1 because the relation between mean surface temperature , Nusselt number and convective heat flux is not unique .
	manualset3
87387	6	398694	13	NULL	NULL	0	NULL	 4 m s-1 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , a bulk Nesselt number should not be used to estimate heat loss from a live sheep in a hot environment if the windspeed is below about 4 m s-1 because the relation between mean surface temperature , Nusselt number and convective heat flux is not unique .
	manualset3
87388	7	398694	13	NULL	NULL	0	NULL	mean surface temperature	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , a bulk Nesselt number should not be used to estimate heat loss from a live sheep in a hot environment if the windspeed is below about 4 m s-1 because the relation between mean surface temperature , Nusselt number and convective heat flux is not unique .
	manualset3
87389	8	398694	13	NULL	NULL	NULL	NULL	Nusselt number	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , a bulk Nesselt number should not be used to estimate heat loss from a live sheep in a hot environment if the windspeed is below about 4 m s-1 because the relation between mean surface temperature , Nusselt number and convective heat flux is not unique .
	manualset3
87390	9	398694	13	NULL	NULL	0	NULL	convective heat flux	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , a bulk Nesselt number should not be used to estimate heat loss from a live sheep in a hot environment if the windspeed is below about 4 m s-1 because the relation between mean surface temperature , Nusselt number and convective heat flux is not unique .
	manualset3
87391	1	398695	13	NULL	NULL	NULL	NULL	onset of caudal cranial nerve symptoms	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , a case with a sudden onset of caudal cranial nerve symptoms , before evident symptoms due to subarachnoid hemorrhage , has never been reported previously .
	manualset3
87392	2	398695	13	NULL	NULL	NULL	NULL	symptoms due to subarachnoid hemorrhage	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , a case with a sudden onset of caudal cranial nerve symptoms , before evident symptoms due to subarachnoid hemorrhage , has never been reported previously .
	manualset3
87393	1	398696	13	NULL	NULL	0	NULL	ALVAC-GM-CSF	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , a combination of ALVAC-GM-CSF and ALVAC-IL12 had no synergistic effect .
	manualset3
87394	2	398696	13	NULL	NULL	0	NULL	ALVAC-IL12	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , a combination of ALVAC-GM-CSF and ALVAC-IL12 had no synergistic effect .
	manualset3
87395	1	398697	13	NULL	NULL	0	NULL	reliance	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , a concern with reliance upon steady-state drug concentrations is that it ignores events occurring while the pathogen is exposed to intermittent suboptimal systemic drug concentrations prior to the attainment of a steady state .
	manualset3
87396	2	398697	13	NULL	NULL	NULL	NULL	steady-state drug concentrations	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , a concern with reliance upon steady-state drug concentrations is that it ignores events occurring while the pathogen is exposed to intermittent suboptimal systemic drug concentrations prior to the attainment of a steady state .
	manualset3
87397	3	398697	13	NULL	NULL	0	NULL	 pathogen 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , a concern with reliance upon steady-state drug concentrations is that it ignores events occurring while the pathogen is exposed to intermittent suboptimal systemic drug concentrations prior to the attainment of a steady state .
	manualset3
87398	4	398697	13	NULL	NULL	NULL	NULL	suboptimal systemic drug concentrations 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , a concern with reliance upon steady-state drug concentrations is that it ignores events occurring while the pathogen is exposed to intermittent suboptimal systemic drug concentrations prior to the attainment of a steady state .
	manualset3
87399	5	398697	13	NULL	NULL	NULL	NULL	steady state	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , a concern with reliance upon steady-state drug concentrations is that it ignores events occurring while the pathogen is exposed to intermittent suboptimal systemic drug concentrations prior to the attainment of a steady state .
	manualset3
87400	1	398698	13	NULL	NULL	0	NULL	evidence 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , a growing body of evidence suggests that intracellular peptide hormone , either internalized or synthesized in situ , can exert physiologically relevant effects .
	manualset3
87401	2	398698	13	NULL	NULL	0	NULL	peptide hormone	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , a growing body of evidence suggests that intracellular peptide hormone , either internalized or synthesized in situ , can exert physiologically relevant effects .
	manualset3
87402	3	398698	13	NULL	NULL	NULL	NULL	internalized 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , a growing body of evidence suggests that intracellular peptide hormone , either internalized or synthesized in situ , can exert physiologically relevant effects .
	manualset3
87403	4	398698	13	NULL	NULL	0	NULL	synthesized 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , a growing body of evidence suggests that intracellular peptide hormone , either internalized or synthesized in situ , can exert physiologically relevant effects .
	manualset3
87404	1	398699	13	NULL	NULL	0	NULL	null mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , a likely null mutation in the Shab K ( + ) channel gene ( Shab ( 3 ) ) reduces I ( K ) but does not eliminate it .
	manualset3
87405	2	398699	13	NULL	NULL	0	NULL	Shab K ( + ) channel gene ( Shab ( 3 ) )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	However , a likely null mutation in the Shab K ( + ) channel gene ( Shab ( 3 ) ) reduces I ( K ) but does not eliminate it .
	manualset3
87406	3	398699	13	NULL	NULL	0	NULL	I ( K )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , a likely null mutation in the Shab K ( + ) channel gene ( Shab ( 3 ) ) reduces I ( K ) but does not eliminate it .
	manualset3
87407	1	398700	13	NULL	NULL	0	NULL	tunicamycin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , a possible effect of tunicamycin on the expression of the Ca channel as an alternative mechanism can not be excluded .
	manualset3
87408	2	398700	13	NULL	NULL	0	NULL	expression of the Ca channel	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , a possible effect of tunicamycin on the expression of the Ca channel as an alternative mechanism can not be excluded .
	manualset3
87409	3	398700	13	NULL	NULL	0	NULL	mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , a possible effect of tunicamycin on the expression of the Ca channel as an alternative mechanism can not be excluded .
	manualset3
87410	1	398701	13	NULL	NULL	0	NULL	 24-h recording period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	However , across the 24-h recording period IL-6 knockout mice spent approximately 30 % more time in rapid eye movements sleep ( REMS ) than did C57BL/6J mice .
	manualset3
87411	2	398701	13	NULL	NULL	0	NULL	IL-6 knockout mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , across the 24-h recording period IL-6 knockout mice spent approximately 30 % more time in rapid eye movements sleep ( REMS ) than did C57BL/6J mice .
	manualset3
87412	3	398701	13	NULL	NULL	0	NULL	30 % more time 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , across the 24-h recording period IL-6 knockout mice spent approximately 30 % more time in rapid eye movements sleep ( REMS ) than did C57BL/6J mice .
	manualset3
87413	4	398701	13	NULL	NULL	0	NULL	rapid eye movements sleep ( REMS ) 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , across the 24-h recording period IL-6 knockout mice spent approximately 30 % more time in rapid eye movements sleep ( REMS ) than did C57BL/6J mice .
	manualset3
87414	5	398701	13	NULL	NULL	0	NULL	C57BL/6J mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , across the 24-h recording period IL-6 knockout mice spent approximately 30 % more time in rapid eye movements sleep ( REMS ) than did C57BL/6J mice .
	manualset3
87415	1	398702	13	NULL	NULL	0	NULL	activation of p53	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , activation of p53 was suppressed by SP600125 ; therefore the function of p53 was possibly controlled by JNK as well .
	manualset3
87416	2	398702	13	NULL	NULL	0	NULL	SP600125	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , activation of p53 was suppressed by SP600125 ; therefore the function of p53 was possibly controlled by JNK as well .
	manualset3
87417	3	398702	13	NULL	NULL	0	NULL	function of p53	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , activation of p53 was suppressed by SP600125 ; therefore the function of p53 was possibly controlled by JNK as well .
	manualset3
87418	4	398702	13	NULL	NULL	0	NULL	JNK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , activation of p53 was suppressed by SP600125 ; therefore the function of p53 was possibly controlled by JNK as well .
	manualset3
87419	1	398703	13	NULL	NULL	0	NULL	acute tubular necrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , acute tubular necrosis was present both in IR non-treated and IR+FTY 720-treated groups .
	manualset3
87420	2	398703	13	NULL	NULL	NULL	NULL	IR non-treated group	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , acute tubular necrosis was present both in IR non-treated and IR+FTY 720-treated groups .
	manualset3
87421	3	398703	13	NULL	NULL	NULL	NULL	IR+FTY 720-treated group	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , acute tubular necrosis was present both in IR non-treated and IR+FTY 720-treated groups .
	manualset3
87422	1	398704	13	NULL	NULL	NULL	NULL	ischemia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , after in vitro ischemia on hippocampal slices , both EAAs and PEA concentrations increased , but with different temporal patterns .
	manualset3
87423	2	398704	13	NULL	NULL	0	NULL	hippocampal slices	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , after in vitro ischemia on hippocampal slices , both EAAs and PEA concentrations increased , but with different temporal patterns .
	manualset3
87424	3	398704	13	NULL	NULL	0	NULL	EAAs	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	However , after in vitro ischemia on hippocampal slices , both EAAs and PEA concentrations increased , but with different temporal patterns .
	manualset3
87425	4	398704	13	NULL	NULL	0	NULL	PEA	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , after in vitro ischemia on hippocampal slices , both EAAs and PEA concentrations increased , but with different temporal patterns .
	manualset3
87426	5	398704	13	NULL	NULL	0	NULL	 temporal patterns	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , after in vitro ischemia on hippocampal slices , both EAAs and PEA concentrations increased , but with different temporal patterns .
	manualset3
87427	1	398705	13	NULL	NULL	0	NULL	indomethacin administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , after indomethacin administration , only hypertensive patients showed a significant reduction in the 24-hour sodium excretion ( from 417 + / - 61 to 317 + / - 49 mEq , p less than 0.05 ) , so that the difference between this value and the corresponding value of normotensive subjects ( 453 + / - 79 mEq ) became significant ( p less than 0.05 ) .
	manualset3
87428	2	398705	13	NULL	NULL	0	NULL	hypertensive patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , after indomethacin administration , only hypertensive patients showed a significant reduction in the 24-hour sodium excretion ( from 417 + / - 61 to 317 + / - 49 mEq , p less than 0.05 ) , so that the difference between this value and the corresponding value of normotensive subjects ( 453 + / - 79 mEq ) became significant ( p less than 0.05 ) .
	manualset3
87429	3	398705	13	NULL	NULL	0	NULL	24-hour	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	However , after indomethacin administration , only hypertensive patients showed a significant reduction in the 24-hour sodium excretion ( from 417 + / - 61 to 317 + / - 49 mEq , p less than 0.05 ) , so that the difference between this value and the corresponding value of normotensive subjects ( 453 + / - 79 mEq ) became significant ( p less than 0.05 ) .
	manualset3
87430	4	398705	13	NULL	NULL	0	NULL	sodium excretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , after indomethacin administration , only hypertensive patients showed a significant reduction in the 24-hour sodium excretion ( from 417 + / - 61 to 317 + / - 49 mEq , p less than 0.05 ) , so that the difference between this value and the corresponding value of normotensive subjects ( 453 + / - 79 mEq ) became significant ( p less than 0.05 ) .
	manualset3
87431	5	398705	13	NULL	NULL	NULL	NULL	417 + / - 61 to 317 + / - 49 mEq 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , after indomethacin administration , only hypertensive patients showed a significant reduction in the 24-hour sodium excretion ( from 417 + / - 61 to 317 + / - 49 mEq , p less than 0.05 ) , so that the difference between this value and the corresponding value of normotensive subjects ( 453 + / - 79 mEq ) became significant ( p less than 0.05 ) .
	manualset3
87432	6	398705	13	NULL	NULL	0	NULL	normotensive subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , after indomethacin administration , only hypertensive patients showed a significant reduction in the 24-hour sodium excretion ( from 417 + / - 61 to 317 + / - 49 mEq , p less than 0.05 ) , so that the difference between this value and the corresponding value of normotensive subjects ( 453 + / - 79 mEq ) became significant ( p less than 0.05 ) .
	manualset3
87433	7	398705	13	NULL	NULL	0	NULL	453 + / - 79 mEq	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , after indomethacin administration , only hypertensive patients showed a significant reduction in the 24-hour sodium excretion ( from 417 + / - 61 to 317 + / - 49 mEq , p less than 0.05 ) , so that the difference between this value and the corresponding value of normotensive subjects ( 453 + / - 79 mEq ) became significant ( p less than 0.05 ) .
	manualset3
87434	8	398705	13	NULL	NULL	0	NULL	p less than 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , after indomethacin administration , only hypertensive patients showed a significant reduction in the 24-hour sodium excretion ( from 417 + / - 61 to 317 + / - 49 mEq , p less than 0.05 ) , so that the difference between this value and the corresponding value of normotensive subjects ( 453 + / - 79 mEq ) became significant ( p less than 0.05 ) .
	manualset3
89563	9	398705	13	NULL	NULL	0	NULL	p less than 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , after indomethacin administration , only hypertensive patients showed a significant reduction in the 24-hour sodium excretion ( from 417 + / - 61 to 317 + / - 49 mEq , p less than 0.05 ) , so that the difference between this value and the corresponding value of normotensive subjects ( 453 + / - 79 mEq ) became significant ( p less than 0.05 ) .
	manualset3
87435	1	398706	13	NULL	NULL	0	NULL	urethane treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , after urethane treatment , most strains carrying the Pas1 ( s ) allele show an intermediate ( 1-4 tumors/mouse ) instead of a highly susceptible ( 15-30 tumors/mouse ) lung tumor phenotype .
	manualset3
87436	2	398706	13	NULL	NULL	0	NULL	strains carrying the Pas1 ( s ) allele	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , after urethane treatment , most strains carrying the Pas1 ( s ) allele show an intermediate ( 1-4 tumors/mouse ) instead of a highly susceptible ( 15-30 tumors/mouse ) lung tumor phenotype .
	manualset3
87437	3	398706	13	NULL	NULL	0	NULL	 intermediate ( 1-4 tumors/mouse ) lung tumor phenotype 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , after urethane treatment , most strains carrying the Pas1 ( s ) allele show an intermediate ( 1-4 tumors/mouse ) instead of a highly susceptible ( 15-30 tumors/mouse ) lung tumor phenotype .
	manualset3
87438	4	398706	13	NULL	NULL	0	NULL	highly susceptible ( 15-30 tumors/mouse ) lung tumor phenotype 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , after urethane treatment , most strains carrying the Pas1 ( s ) allele show an intermediate ( 1-4 tumors/mouse ) instead of a highly susceptible ( 15-30 tumors/mouse ) lung tumor phenotype .
	manualset3
87439	1	398707	13	NULL	NULL	NULL	NULL	non-esterified fatty acid parameters	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , all non-esterified fatty acid parameters showed only modest inverse correlation with liver transaminases .
	manualset3
87440	2	398707	13	NULL	NULL	NULL	NULL	modest inverse correlation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , all non-esterified fatty acid parameters showed only modest inverse correlation with liver transaminases .
	manualset3
87441	3	398707	13	NULL	NULL	NULL	NULL	liver transaminases	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , all non-esterified fatty acid parameters showed only modest inverse correlation with liver transaminases .
	manualset3
87442	1	398708	13	NULL	NULL	0	NULL	analytes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , analytes that form protonated molecular ions , such as reserpine , also show higher signal intensities when a ground loop is introduced into the system .
	manualset3
87443	2	398708	13	NULL	NULL	NULL	NULL	protonated molecular ions	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , analytes that form protonated molecular ions , such as reserpine , also show higher signal intensities when a ground loop is introduced into the system .
	manualset3
87444	3	398708	13	NULL	NULL	0	NULL	 reserpine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , analytes that form protonated molecular ions , such as reserpine , also show higher signal intensities when a ground loop is introduced into the system .
	manualset3
87445	4	398708	13	NULL	NULL	0	NULL	ground loop	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	However , analytes that form protonated molecular ions , such as reserpine , also show higher signal intensities when a ground loop is introduced into the system .
	manualset3
87446	5	398708	13	NULL	NULL	0	NULL	system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	However , analytes that form protonated molecular ions , such as reserpine , also show higher signal intensities when a ground loop is introduced into the system .
	manualset3
87447	1	398709	13	NULL	NULL	0	NULL	androgens 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , androgens are not widely used for these indications because of the side effects associated with these drugs .
	manualset3
87448	2	398709	13	NULL	NULL	0	NULL	 indications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , androgens are not widely used for these indications because of the side effects associated with these drugs .
	manualset3
87449	3	398709	13	NULL	NULL	0	NULL	side effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , androgens are not widely used for these indications because of the side effects associated with these drugs .
	manualset3
87450	4	398709	13	NULL	NULL	0	NULL	drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , androgens are not widely used for these indications because of the side effects associated with these drugs .
	manualset3
87451	1	398710	13	NULL	NULL	NULL	NULL	antisense ODN-mediated depletion of mitogen-activated protein kinases	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , antisense ODN-mediated depletion of mitogen-activated protein kinases from the cells showed that their expression was necessary for terminal differentiation .
	manualset3
87452	2	398710	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , antisense ODN-mediated depletion of mitogen-activated protein kinases from the cells showed that their expression was necessary for terminal differentiation .
	manualset3
87453	3	398710	13	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , antisense ODN-mediated depletion of mitogen-activated protein kinases from the cells showed that their expression was necessary for terminal differentiation .
	manualset3
87454	4	398710	13	NULL	NULL	0	NULL	terminal differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , antisense ODN-mediated depletion of mitogen-activated protein kinases from the cells showed that their expression was necessary for terminal differentiation .
	manualset3
87455	1	398711	13	NULL	NULL	0	NULL	central thermoregulatory action	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( The central thermoregulatory action of cholecystokinin-8 and prostaglandin E1 ) .
	manualset3
87456	2	398711	13	NULL	NULL	0	NULL	cholecystokinin-8 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( The central thermoregulatory action of cholecystokinin-8 and prostaglandin E1 ) .
	manualset3
87457	3	398711	13	NULL	NULL	0	NULL	prostaglandin E1	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( The central thermoregulatory action of cholecystokinin-8 and prostaglandin E1 ) .
	manualset3
87458	1	398712	13	NULL	NULL	0	NULL	membrane-interacting agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , application of membrane-interacting agents like tris ( hydroxymethyl ) aminomethane ( Tris ) - hydrochloride , ethylenediaminetetraacetate ( Na salt ) ( EDTA ) , divalent cations , and sublethal doses of the cationic antibacterial agents polymyxin B and chlorhexidine induced specific fluorescent labeling of envelope proteins and lipids but not of cytoplasmic compounds , with the exception of a soluble protein with a molecular weight of 46 , 000 in sodium dodecyl sulfate-polyacrylamide gel electrophoresis .
	manualset3
87459	2	398712	13	NULL	NULL	NULL	NULL	tris ( hydroxymethyl ) aminomethane ( Tris ) - hydrochloride	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , application of membrane-interacting agents like tris ( hydroxymethyl ) aminomethane ( Tris ) - hydrochloride , ethylenediaminetetraacetate ( Na salt ) ( EDTA ) , divalent cations , and sublethal doses of the cationic antibacterial agents polymyxin B and chlorhexidine induced specific fluorescent labeling of envelope proteins and lipids but not of cytoplasmic compounds , with the exception of a soluble protein with a molecular weight of 46 , 000 in sodium dodecyl sulfate-polyacrylamide gel electrophoresis .
	manualset3
87460	3	398712	13	NULL	NULL	0	NULL	ethylenediaminetetraacetate ( Na salt ) ( EDTA ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , application of membrane-interacting agents like tris ( hydroxymethyl ) aminomethane ( Tris ) - hydrochloride , ethylenediaminetetraacetate ( Na salt ) ( EDTA ) , divalent cations , and sublethal doses of the cationic antibacterial agents polymyxin B and chlorhexidine induced specific fluorescent labeling of envelope proteins and lipids but not of cytoplasmic compounds , with the exception of a soluble protein with a molecular weight of 46 , 000 in sodium dodecyl sulfate-polyacrylamide gel electrophoresis .
	manualset3
87461	4	398712	13	NULL	NULL	0	NULL	divalent cations 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	However , application of membrane-interacting agents like tris ( hydroxymethyl ) aminomethane ( Tris ) - hydrochloride , ethylenediaminetetraacetate ( Na salt ) ( EDTA ) , divalent cations , and sublethal doses of the cationic antibacterial agents polymyxin B and chlorhexidine induced specific fluorescent labeling of envelope proteins and lipids but not of cytoplasmic compounds , with the exception of a soluble protein with a molecular weight of 46 , 000 in sodium dodecyl sulfate-polyacrylamide gel electrophoresis .
	manualset3
87462	5	398712	13	NULL	NULL	NULL	NULL	cationic antibacterial agents 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , application of membrane-interacting agents like tris ( hydroxymethyl ) aminomethane ( Tris ) - hydrochloride , ethylenediaminetetraacetate ( Na salt ) ( EDTA ) , divalent cations , and sublethal doses of the cationic antibacterial agents polymyxin B and chlorhexidine induced specific fluorescent labeling of envelope proteins and lipids but not of cytoplasmic compounds , with the exception of a soluble protein with a molecular weight of 46 , 000 in sodium dodecyl sulfate-polyacrylamide gel electrophoresis .
	manualset3
87463	6	398712	13	NULL	NULL	0	NULL	polymyxin B	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , application of membrane-interacting agents like tris ( hydroxymethyl ) aminomethane ( Tris ) - hydrochloride , ethylenediaminetetraacetate ( Na salt ) ( EDTA ) , divalent cations , and sublethal doses of the cationic antibacterial agents polymyxin B and chlorhexidine induced specific fluorescent labeling of envelope proteins and lipids but not of cytoplasmic compounds , with the exception of a soluble protein with a molecular weight of 46 , 000 in sodium dodecyl sulfate-polyacrylamide gel electrophoresis .
	manualset3
87464	7	398712	13	NULL	NULL	0	NULL	chlorhexidine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , application of membrane-interacting agents like tris ( hydroxymethyl ) aminomethane ( Tris ) - hydrochloride , ethylenediaminetetraacetate ( Na salt ) ( EDTA ) , divalent cations , and sublethal doses of the cationic antibacterial agents polymyxin B and chlorhexidine induced specific fluorescent labeling of envelope proteins and lipids but not of cytoplasmic compounds , with the exception of a soluble protein with a molecular weight of 46 , 000 in sodium dodecyl sulfate-polyacrylamide gel electrophoresis .
	manualset3
87465	8	398712	13	NULL	NULL	0	NULL	specific fluorescent labeling of envelope proteins and lipids	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , application of membrane-interacting agents like tris ( hydroxymethyl ) aminomethane ( Tris ) - hydrochloride , ethylenediaminetetraacetate ( Na salt ) ( EDTA ) , divalent cations , and sublethal doses of the cationic antibacterial agents polymyxin B and chlorhexidine induced specific fluorescent labeling of envelope proteins and lipids but not of cytoplasmic compounds , with the exception of a soluble protein with a molecular weight of 46 , 000 in sodium dodecyl sulfate-polyacrylamide gel electrophoresis .
	manualset3
87466	9	398712	13	NULL	NULL	0	NULL	cytoplasmic compounds	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , application of membrane-interacting agents like tris ( hydroxymethyl ) aminomethane ( Tris ) - hydrochloride , ethylenediaminetetraacetate ( Na salt ) ( EDTA ) , divalent cations , and sublethal doses of the cationic antibacterial agents polymyxin B and chlorhexidine induced specific fluorescent labeling of envelope proteins and lipids but not of cytoplasmic compounds , with the exception of a soluble protein with a molecular weight of 46 , 000 in sodium dodecyl sulfate-polyacrylamide gel electrophoresis .
	manualset3
87467	10	398712	13	NULL	NULL	0	NULL	soluble protein with a molecular weight of 46 , 000 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , application of membrane-interacting agents like tris ( hydroxymethyl ) aminomethane ( Tris ) - hydrochloride , ethylenediaminetetraacetate ( Na salt ) ( EDTA ) , divalent cations , and sublethal doses of the cationic antibacterial agents polymyxin B and chlorhexidine induced specific fluorescent labeling of envelope proteins and lipids but not of cytoplasmic compounds , with the exception of a soluble protein with a molecular weight of 46 , 000 in sodium dodecyl sulfate-polyacrylamide gel electrophoresis .
	manualset3
87468	11	398712	13	NULL	NULL	0	NULL	sodium dodecyl sulfate-polyacrylamide gel electrophoresis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , application of membrane-interacting agents like tris ( hydroxymethyl ) aminomethane ( Tris ) - hydrochloride , ethylenediaminetetraacetate ( Na salt ) ( EDTA ) , divalent cations , and sublethal doses of the cationic antibacterial agents polymyxin B and chlorhexidine induced specific fluorescent labeling of envelope proteins and lipids but not of cytoplasmic compounds , with the exception of a soluble protein with a molecular weight of 46 , 000 in sodium dodecyl sulfate-polyacrylamide gel electrophoresis .
	manualset3
89566	12	398712	13	NULL	NULL	0	NULL	sublethal doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , application of membrane-interacting agents like tris ( hydroxymethyl ) aminomethane ( Tris ) - hydrochloride , ethylenediaminetetraacetate ( Na salt ) ( EDTA ) , divalent cations , and sublethal doses of the cationic antibacterial agents polymyxin B and chlorhexidine induced specific fluorescent labeling of envelope proteins and lipids but not of cytoplasmic compounds , with the exception of a soluble protein with a molecular weight of 46 , 000 in sodium dodecyl sulfate-polyacrylamide gel electrophoresis .
	manualset3
87469	1	398713	13	NULL	NULL	0	NULL	apyrase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , apyrase , an ATPase and ADPase , did not inhibit the shear-induced ( Ca2 + ) i responses in standard medium ( no added ATP or ADP ) , suggesting that the shear-induced ( Ca2 + ) i response is not due to ATP released by endothelial cells .
	manualset3
87470	2	398713	13	NULL	NULL	0	NULL	ATPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , apyrase , an ATPase and ADPase , did not inhibit the shear-induced ( Ca2 + ) i responses in standard medium ( no added ATP or ADP ) , suggesting that the shear-induced ( Ca2 + ) i response is not due to ATP released by endothelial cells .
	manualset3
87471	3	398713	13	NULL	NULL	0	NULL	ADPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , apyrase , an ATPase and ADPase , did not inhibit the shear-induced ( Ca2 + ) i responses in standard medium ( no added ATP or ADP ) , suggesting that the shear-induced ( Ca2 + ) i response is not due to ATP released by endothelial cells .
	manualset3
87472	4	398713	13	NULL	NULL	0	NULL	shear-induced ( Ca2 + ) i responses 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , apyrase , an ATPase and ADPase , did not inhibit the shear-induced ( Ca2 + ) i responses in standard medium ( no added ATP or ADP ) , suggesting that the shear-induced ( Ca2 + ) i response is not due to ATP released by endothelial cells .
	manualset3
87473	5	398713	13	NULL	NULL	0	NULL	standard medium ( no added ATP or ADP )	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , apyrase , an ATPase and ADPase , did not inhibit the shear-induced ( Ca2 + ) i responses in standard medium ( no added ATP or ADP ) , suggesting that the shear-induced ( Ca2 + ) i response is not due to ATP released by endothelial cells .
	manualset3
87474	6	398713	13	NULL	NULL	0	NULL	shear-induced ( Ca2 + ) i response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , apyrase , an ATPase and ADPase , did not inhibit the shear-induced ( Ca2 + ) i responses in standard medium ( no added ATP or ADP ) , suggesting that the shear-induced ( Ca2 + ) i response is not due to ATP released by endothelial cells .
	manualset3
87475	7	398713	13	NULL	NULL	0	NULL	ATP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , apyrase , an ATPase and ADPase , did not inhibit the shear-induced ( Ca2 + ) i responses in standard medium ( no added ATP or ADP ) , suggesting that the shear-induced ( Ca2 + ) i response is not due to ATP released by endothelial cells .
	manualset3
87476	8	398713	13	NULL	NULL	0	NULL	endothelial cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , apyrase , an ATPase and ADPase , did not inhibit the shear-induced ( Ca2 + ) i responses in standard medium ( no added ATP or ADP ) , suggesting that the shear-induced ( Ca2 + ) i response is not due to ATP released by endothelial cells .
	manualset3
87477	1	398714	13	NULL	NULL	0	NULL	 frontal electrodes	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	However , at the frontal electrodes , late positivity ( probably a P3a ) only appeared in valid-invalid trials , indicating that invalid trials are analyzed as novel-like stimuli .
	manualset3
87478	2	398714	13	NULL	NULL	0	NULL	valid-invalid trials	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , at the frontal electrodes , late positivity ( probably a P3a ) only appeared in valid-invalid trials , indicating that invalid trials are analyzed as novel-like stimuli .
	manualset3
87479	3	398714	13	NULL	NULL	0	NULL	invalid trials are analyzed	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , at the frontal electrodes , late positivity ( probably a P3a ) only appeared in valid-invalid trials , indicating that invalid trials are analyzed as novel-like stimuli .
	manualset3
87480	4	398714	13	NULL	NULL	0	NULL	novel-like stimuli	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , at the frontal electrodes , late positivity ( probably a P3a ) only appeared in valid-invalid trials , indicating that invalid trials are analyzed as novel-like stimuli .
	manualset3
87481	1	398715	13	NULL	NULL	0	NULL	( 1 microM ) NT ( 8-13 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , at the highest concentration studied ( 1 microM ) NT ( 8-13 ) was associated with a rapid increase ( 130 % ) in striatal dopamine release .
	manualset3
87482	2	398715	13	NULL	NULL	0	NULL	130 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , at the highest concentration studied ( 1 microM ) NT ( 8-13 ) was associated with a rapid increase ( 130 % ) in striatal dopamine release .
	manualset3
87483	3	398715	13	NULL	NULL	0	NULL	striatal dopamine release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , at the highest concentration studied ( 1 microM ) NT ( 8-13 ) was associated with a rapid increase ( 130 % ) in striatal dopamine release .
	manualset3
87484	1	398716	13	NULL	NULL	0	NULL	clomipramine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , because clomipramine is an effective treatment , information about the drug 's neurochemical effect could enhance the understanding of canine CD .
	manualset3
87485	2	398716	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , because clomipramine is an effective treatment , information about the drug 's neurochemical effect could enhance the understanding of canine CD .
	manualset3
87486	3	398716	13	NULL	NULL	0	NULL	drug 's neurochemical effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , because clomipramine is an effective treatment , information about the drug 's neurochemical effect could enhance the understanding of canine CD .
	manualset3
87487	4	398716	13	NULL	NULL	0	NULL	canine CD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	However , because clomipramine is an effective treatment , information about the drug 's neurochemical effect could enhance the understanding of canine CD .
	manualset3
87488	1	398717	13	NULL	NULL	0	NULL	 29 and 84 ( early milking phase ) 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	However , between d 29 and 84 ( early milking phase ) , mean daily milk yield was greater in LD1X does than in DD1X does ( 2.6 0.1 kg vs. 2.1 0.1 kg ; P = 0.001 ) .
	manualset3
87489	2	398717	13	NULL	NULL	0	NULL	mean daily milk yield	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , between d 29 and 84 ( early milking phase ) , mean daily milk yield was greater in LD1X does than in DD1X does ( 2.6 0.1 kg vs. 2.1 0.1 kg ; P = 0.001 ) .
	manualset3
87490	3	398717	13	NULL	NULL	0	NULL	LD1X	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , between d 29 and 84 ( early milking phase ) , mean daily milk yield was greater in LD1X does than in DD1X does ( 2.6 0.1 kg vs. 2.1 0.1 kg ; P = 0.001 ) .
	manualset3
87491	4	398717	13	NULL	NULL	0	NULL	 DD1X 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , between d 29 and 84 ( early milking phase ) , mean daily milk yield was greater in LD1X does than in DD1X does ( 2.6 0.1 kg vs. 2.1 0.1 kg ; P = 0.001 ) .
	manualset3
87492	5	398717	13	NULL	NULL	0	NULL	( 2.6 0.1 kg vs. 2.1 0.1 kg ; P = 0.001 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , between d 29 and 84 ( early milking phase ) , mean daily milk yield was greater in LD1X does than in DD1X does ( 2.6 0.1 kg vs. 2.1 0.1 kg ; P = 0.001 ) .
	manualset3
87493	1	398718	13	NULL	NULL	0	NULL	meaning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , both meaning and forgiveness conferred mental health benefits for all three groups .
	manualset3
87494	2	398718	13	NULL	NULL	0	NULL	forgiveness 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , both meaning and forgiveness conferred mental health benefits for all three groups .
	manualset3
87495	3	398718	13	NULL	NULL	0	NULL	mental health benefits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , both meaning and forgiveness conferred mental health benefits for all three groups .
	manualset3
87496	4	398718	13	NULL	NULL	0	NULL	three groups	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , both meaning and forgiveness conferred mental health benefits for all three groups .
	manualset3
87497	1	398719	13	NULL	NULL	0	NULL	D137-L 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , both D137-L and E139-L had fusion activities equivalent to that of wild-type G protein after exposure to a pH of 5.7 or below .
	manualset3
87498	2	398719	13	NULL	NULL	0	NULL	E139-L	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , both D137-L and E139-L had fusion activities equivalent to that of wild-type G protein after exposure to a pH of 5.7 or below .
	manualset3
87499	3	398719	13	NULL	NULL	0	NULL	wild-type G protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , both D137-L and E139-L had fusion activities equivalent to that of wild-type G protein after exposure to a pH of 5.7 or below .
	manualset3
87500	4	398719	13	NULL	NULL	NULL	NULL	exposure 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , both D137-L and E139-L had fusion activities equivalent to that of wild-type G protein after exposure to a pH of 5.7 or below .
	manualset3
87719	5	398719	13	NULL	NULL	0	NULL	pH of 5.7 or below	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , both D137-L and E139-L had fusion activities equivalent to that of wild-type G protein after exposure to a pH of 5.7 or below .
	manualset3
87501	1	398720	13	NULL	NULL	0	NULL	radioprotectant B-190	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( The characteristic of radioprotective properties of a radioprotectant B-190 at its administration after radiation ) .
	manualset3
87502	2	398720	13	NULL	NULL	NULL	NULL	administration 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The characteristic of radioprotective properties of a radioprotectant B-190 at its administration after radiation ) .
	manualset3
87503	3	398720	13	NULL	NULL	0	NULL	 radiation 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	( The characteristic of radioprotective properties of a radioprotectant B-190 at its administration after radiation ) .
	manualset3
87504	1	398721	13	NULL	NULL	NULL	NULL	stimuli	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , both forms of stimuli also activate other receptors .
	manualset3
87505	2	398721	13	NULL	NULL	0	NULL	activate other receptors	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , both forms of stimuli also activate other receptors .
	manualset3
87506	1	398722	13	NULL	NULL	NULL	NULL	80 pg/ml	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , by adding 80 pg/ml naloxone to the culture system containing 600 pg/ml beta-endorphin , the inhibitory effect of beta-endorphin on spontaneous GVBD could be reversed completely .
	manualset3
87507	2	398722	13	NULL	NULL	0	NULL	naloxone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , by adding 80 pg/ml naloxone to the culture system containing 600 pg/ml beta-endorphin , the inhibitory effect of beta-endorphin on spontaneous GVBD could be reversed completely .
	manualset3
87508	3	398722	13	NULL	NULL	0	NULL	culture system	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , by adding 80 pg/ml naloxone to the culture system containing 600 pg/ml beta-endorphin , the inhibitory effect of beta-endorphin on spontaneous GVBD could be reversed completely .
	manualset3
87509	4	398722	13	NULL	NULL	NULL	NULL	600 pg/ml 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , by adding 80 pg/ml naloxone to the culture system containing 600 pg/ml beta-endorphin , the inhibitory effect of beta-endorphin on spontaneous GVBD could be reversed completely .
	manualset3
87510	5	398722	13	NULL	NULL	0	NULL	beta-endorphin	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	However , by adding 80 pg/ml naloxone to the culture system containing 600 pg/ml beta-endorphin , the inhibitory effect of beta-endorphin on spontaneous GVBD could be reversed completely .
	manualset3
87511	6	398722	13	NULL	NULL	0	NULL	beta-endorphin	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	However , by adding 80 pg/ml naloxone to the culture system containing 600 pg/ml beta-endorphin , the inhibitory effect of beta-endorphin on spontaneous GVBD could be reversed completely .
	manualset3
87512	7	398722	13	NULL	NULL	NULL	NULL	GVBD	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , by adding 80 pg/ml naloxone to the culture system containing 600 pg/ml beta-endorphin , the inhibitory effect of beta-endorphin on spontaneous GVBD could be reversed completely .
	manualset3
87513	1	398723	13	NULL	NULL	NULL	NULL	 zyxin SNP	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , by single marker association , several of the zyxin SNP were significantly associated with carotenoid or NO ( 2 ) ( - ) + NO ( 3 ) ( - ) concentrations .
	manualset3
87514	2	398723	13	NULL	NULL	0	NULL	carotenoid	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , by single marker association , several of the zyxin SNP were significantly associated with carotenoid or NO ( 2 ) ( - ) + NO ( 3 ) ( - ) concentrations .
	manualset3
87515	3	398723	13	NULL	NULL	0	NULL	NO ( 2 ) ( - ) + NO ( 3 ) ( - )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	However , by single marker association , several of the zyxin SNP were significantly associated with carotenoid or NO ( 2 ) ( - ) + NO ( 3 ) ( - ) concentrations .
	manualset3
89567	4	398723	13	NULL	NULL	0	NULL	single marker association	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , by single marker association , several of the zyxin SNP were significantly associated with carotenoid or NO ( 2 ) ( - ) + NO ( 3 ) ( - ) concentrations .
	manualset3
87516	1	398724	13	NULL	NULL	0	NULL	methods of data analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , by supervised methods of data analysis , we were able to select a set of genes that may differentiate between hereditary and sporadic tumors .
	manualset3
87517	2	398724	13	NULL	NULL	0	NULL	set of genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , by supervised methods of data analysis , we were able to select a set of genes that may differentiate between hereditary and sporadic tumors .
	manualset3
87518	3	398724	13	NULL	NULL	0	NULL	hereditary tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , by supervised methods of data analysis , we were able to select a set of genes that may differentiate between hereditary and sporadic tumors .
	manualset3
87519	4	398724	13	NULL	NULL	0	NULL	sporadic tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , by supervised methods of data analysis , we were able to select a set of genes that may differentiate between hereditary and sporadic tumors .
	manualset3
87520	1	398725	13	NULL	NULL	NULL	NULL	techniques	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , by using appropriate techniques , physicians can help patients quit smoking , even when office visits are limited .
	manualset3
87521	2	398725	13	NULL	NULL	0	NULL	physicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , by using appropriate techniques , physicians can help patients quit smoking , even when office visits are limited .
	manualset3
87522	3	398725	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , by using appropriate techniques , physicians can help patients quit smoking , even when office visits are limited .
	manualset3
87523	4	398725	13	NULL	NULL	NULL	NULL	office visits	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , by using appropriate techniques , physicians can help patients quit smoking , even when office visits are limited .
	manualset3
87524	1	398726	13	NULL	NULL	0	NULL	cardiac index	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , cardiac index and left ventricular end-diastolic pressure were unchanged by whole-body cooling .
	manualset3
87525	2	398726	13	NULL	NULL	0	NULL	left ventricular end-diastolic pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , cardiac index and left ventricular end-diastolic pressure were unchanged by whole-body cooling .
	manualset3
87526	3	398726	13	NULL	NULL	NULL	NULL	whole-body 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , cardiac index and left ventricular end-diastolic pressure were unchanged by whole-body cooling .
	manualset3
87527	1	398727	13	NULL	NULL	0	NULL	 changes of transcript patterns	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , causal links between physiological effects and changes of transcript patterns , for the most part , are still unresolved .
	manualset3
87720	2	398727	13	NULL	NULL	0	NULL	causal links 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	However , causal links between physiological effects and changes of transcript patterns , for the most part , are still unresolved .
	manualset3
87721	3	398727	13	NULL	NULL	0	NULL	physiological effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , causal links between physiological effects and changes of transcript patterns , for the most part , are still unresolved .
	manualset3
87528	1	398728	13	NULL	NULL	0	NULL	 interpretation	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , caution should be used in the interpretation of increased cardiovascular disease risk , as it does not necessarily translate into early increased mortality .
	manualset3
87529	2	398728	13	NULL	NULL	0	NULL	cardiovascular disease risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , caution should be used in the interpretation of increased cardiovascular disease risk , as it does not necessarily translate into early increased mortality .
	manualset3
87530	3	398728	13	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , caution should be used in the interpretation of increased cardiovascular disease risk , as it does not necessarily translate into early increased mortality .
	manualset3
87531	1	398729	13	NULL	NULL	NULL	NULL	central anorexigenic action	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , central anorexigenic action of leptin is clearly diminished in aging , most likely due to the impaired leptin signal transduction .
	manualset3
87532	2	398729	13	NULL	NULL	0	NULL	aging	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , central anorexigenic action of leptin is clearly diminished in aging , most likely due to the impaired leptin signal transduction .
	manualset3
87533	3	398729	13	NULL	NULL	0	NULL	leptin signal transduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , central anorexigenic action of leptin is clearly diminished in aging , most likely due to the impaired leptin signal transduction .
	manualset3
87722	4	398729	13	NULL	NULL	0	NULL	leptin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , central anorexigenic action of leptin is clearly diminished in aging , most likely due to the impaired leptin signal transduction .
	manualset3
87723	1	398731	13	NULL	NULL	NULL	NULL	challenges 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , challenges associated with early vascularization of transplanted islet grafts and long-term islet survival remain .
	manualset3
87724	2	398731	13	NULL	NULL	NULL	NULL	early vascularization 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , challenges associated with early vascularization of transplanted islet grafts and long-term islet survival remain .
	manualset3
87725	3	398731	13	NULL	NULL	NULL	NULL	transplanted islet grafts	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , challenges associated with early vascularization of transplanted islet grafts and long-term islet survival remain .
	manualset3
87726	4	398731	13	NULL	NULL	0	NULL	long-term islet survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , challenges associated with early vascularization of transplanted islet grafts and long-term islet survival remain .
	manualset3
87727	1	398732	13	NULL	NULL	NULL	NULL	challenges	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , challenges still lie ahead .
	manualset3
87728	1	398733	13	NULL	NULL	0	NULL	chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , chemotherapy is often cost-prohibitive in our setting as mirrored by limited use ( 17.6 % ) .
	manualset3
87729	2	398733	13	NULL	NULL	0	NULL	17.6 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , chemotherapy is often cost-prohibitive in our setting as mirrored by limited use ( 17.6 % ) .
	manualset3
87730	1	398734	13	NULL	NULL	0	NULL	choline metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , choline metabolism was altered in rats , as indicated by decreases in betaine and increases in phosphocholine with the concomitant induction of betaine-homocysteine methyltransferase and choline kinase gene expression .
	manualset3
87731	2	398734	13	NULL	NULL	0	NULL	 rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , choline metabolism was altered in rats , as indicated by decreases in betaine and increases in phosphocholine with the concomitant induction of betaine-homocysteine methyltransferase and choline kinase gene expression .
	manualset3
87732	3	398734	13	NULL	NULL	NULL	NULL	betaine	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , choline metabolism was altered in rats , as indicated by decreases in betaine and increases in phosphocholine with the concomitant induction of betaine-homocysteine methyltransferase and choline kinase gene expression .
	manualset3
87733	4	398734	13	NULL	NULL	0	NULL	phosphocholine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , choline metabolism was altered in rats , as indicated by decreases in betaine and increases in phosphocholine with the concomitant induction of betaine-homocysteine methyltransferase and choline kinase gene expression .
	manualset3
87734	5	398734	13	NULL	NULL	0	NULL	betaine-homocysteine methyltransferase gene expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , choline metabolism was altered in rats , as indicated by decreases in betaine and increases in phosphocholine with the concomitant induction of betaine-homocysteine methyltransferase and choline kinase gene expression .
	manualset3
87735	6	398734	13	NULL	NULL	0	NULL	choline kinase gene expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , choline metabolism was altered in rats , as indicated by decreases in betaine and increases in phosphocholine with the concomitant induction of betaine-homocysteine methyltransferase and choline kinase gene expression .
	manualset3
87736	1	398735	13	NULL	NULL	0	NULL	clinical cholera infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , clinical cholera infection gave rise to detectable serum antibody responses to soluble hemagglutinin in only 2 of 10 Bangladeshi patients or 1 of 17 cholera-infected North American volunteers .
	manualset3
87737	2	398735	13	NULL	NULL	NULL	NULL	serum antibody responses	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , clinical cholera infection gave rise to detectable serum antibody responses to soluble hemagglutinin in only 2 of 10 Bangladeshi patients or 1 of 17 cholera-infected North American volunteers .
	manualset3
87738	3	398735	13	NULL	NULL	NULL	NULL	soluble hemagglutinin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , clinical cholera infection gave rise to detectable serum antibody responses to soluble hemagglutinin in only 2 of 10 Bangladeshi patients or 1 of 17 cholera-infected North American volunteers .
	manualset3
87739	4	398735	13	NULL	NULL	0	NULL	2 of 10 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , clinical cholera infection gave rise to detectable serum antibody responses to soluble hemagglutinin in only 2 of 10 Bangladeshi patients or 1 of 17 cholera-infected North American volunteers .
	manualset3
87740	5	398735	13	NULL	NULL	0	NULL	Bangladeshi patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , clinical cholera infection gave rise to detectable serum antibody responses to soluble hemagglutinin in only 2 of 10 Bangladeshi patients or 1 of 17 cholera-infected North American volunteers .
	manualset3
87741	6	398735	13	NULL	NULL	0	NULL	1 of 17	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , clinical cholera infection gave rise to detectable serum antibody responses to soluble hemagglutinin in only 2 of 10 Bangladeshi patients or 1 of 17 cholera-infected North American volunteers .
	manualset3
87742	7	398735	13	NULL	NULL	0	NULL	cholera-infected North American volunteers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , clinical cholera infection gave rise to detectable serum antibody responses to soluble hemagglutinin in only 2 of 10 Bangladeshi patients or 1 of 17 cholera-infected North American volunteers .
	manualset3
87743	1	398736	13	NULL	NULL	0	NULL	mRNA expressions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , combining mRNA expressions of genes coding for detoxification enzymes along with enzyme activities will be more useful biomarkers of stress .
	manualset3
87744	2	398736	13	NULL	NULL	0	NULL	genes coding for detoxification enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , combining mRNA expressions of genes coding for detoxification enzymes along with enzyme activities will be more useful biomarkers of stress .
	manualset3
87745	3	398736	13	NULL	NULL	0	NULL	enzyme activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , combining mRNA expressions of genes coding for detoxification enzymes along with enzyme activities will be more useful biomarkers of stress .
	manualset3
87746	4	398736	13	NULL	NULL	0	NULL	biomarkers	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , combining mRNA expressions of genes coding for detoxification enzymes along with enzyme activities will be more useful biomarkers of stress .
	manualset3
87747	5	398736	13	NULL	NULL	NULL	NULL	stress	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , combining mRNA expressions of genes coding for detoxification enzymes along with enzyme activities will be more useful biomarkers of stress .
	manualset3
87748	1	398737	13	NULL	NULL	0	NULL	standard C-Support Vector Machine ( C-SVM )	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	However , comparing to standard C-Support Vector Machine ( C-SVM ) , its formulation is more complicated , up until now there are no effective methods on solving accurate on-line learning for it .
	manualset3
87749	2	398737	13	NULL	NULL	0	NULL	formulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , comparing to standard C-Support Vector Machine ( C-SVM ) , its formulation is more complicated , up until now there are no effective methods on solving accurate on-line learning for it .
	manualset3
87750	3	398737	13	NULL	NULL	NULL	NULL	methods	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , comparing to standard C-Support Vector Machine ( C-SVM ) , its formulation is more complicated , up until now there are no effective methods on solving accurate on-line learning for it .
	manualset3
87751	4	398737	13	NULL	NULL	0	NULL	on-line learning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , comparing to standard C-Support Vector Machine ( C-SVM ) , its formulation is more complicated , up until now there are no effective methods on solving accurate on-line learning for it .
	manualset3
87752	1	398738	13	NULL	NULL	0	NULL	conductance 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , conductance is low when deeply torpid animals are thermo-conforming probably because of peripheral vasoconstriction .
	manualset3
87753	2	398738	13	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , conductance is low when deeply torpid animals are thermo-conforming probably because of peripheral vasoconstriction .
	manualset3
87754	3	398738	13	NULL	NULL	0	NULL	peripheral vasoconstriction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , conductance is low when deeply torpid animals are thermo-conforming probably because of peripheral vasoconstriction .
	manualset3
87755	1	398739	13	NULL	NULL	0	NULL	confusion	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , confusion exists about the purpose of ultrasound scans currently available .
	manualset3
87756	2	398739	13	NULL	NULL	0	NULL	ultrasound scans	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , confusion exists about the purpose of ultrasound scans currently available .
	manualset3
87757	1	398740	13	NULL	NULL	0	NULL	 conservation of synteny	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , conservation of synteny across the cereal genomes , in combination with new maize resources , has now made positional cloning in maize feasible .
	manualset3
87758	2	398740	13	NULL	NULL	NULL	NULL	cereal genomes 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , conservation of synteny across the cereal genomes , in combination with new maize resources , has now made positional cloning in maize feasible .
	manualset3
87759	3	398740	13	NULL	NULL	0	NULL	maize	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , conservation of synteny across the cereal genomes , in combination with new maize resources , has now made positional cloning in maize feasible .
	manualset3
87760	4	398740	13	NULL	NULL	0	NULL	positional cloning	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , conservation of synteny across the cereal genomes , in combination with new maize resources , has now made positional cloning in maize feasible .
	manualset3
87761	5	398740	13	NULL	NULL	0	NULL	maize 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , conservation of synteny across the cereal genomes , in combination with new maize resources , has now made positional cloning in maize feasible .
	manualset3
87762	1	398741	13	NULL	NULL	0	NULL	contributions	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	However , contributions had already appeared in the 1950s showing - albeit indirectly - that isolated mitochondria bound Ca ( 2 + ) actively .
	manualset3
87763	2	398741	13	NULL	NULL	0	NULL	1950s	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	However , contributions had already appeared in the 1950s showing - albeit indirectly - that isolated mitochondria bound Ca ( 2 + ) actively .
	manualset3
87764	3	398741	13	NULL	NULL	0	NULL	mitochondria 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	However , contributions had already appeared in the 1950s showing - albeit indirectly - that isolated mitochondria bound Ca ( 2 + ) actively .
	manualset3
87765	4	398741	13	NULL	NULL	0	NULL	Ca ( 2 + )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	However , contributions had already appeared in the 1950s showing - albeit indirectly - that isolated mitochondria bound Ca ( 2 + ) actively .
	manualset3
87766	1	398742	13	NULL	NULL	0	NULL	 interactions between subunits 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , cooperative interactions between subunits also affect the voltage dependence of channel opening , and these interactions can be altered by making substitutions at uncharged residues in the S4 region .
	manualset3
87767	2	398742	13	NULL	NULL	NULL	NULL	voltage dependence	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , cooperative interactions between subunits also affect the voltage dependence of channel opening , and these interactions can be altered by making substitutions at uncharged residues in the S4 region .
	manualset3
87768	3	398742	13	NULL	NULL	0	NULL	channel opening	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , cooperative interactions between subunits also affect the voltage dependence of channel opening , and these interactions can be altered by making substitutions at uncharged residues in the S4 region .
	manualset3
87769	4	398742	13	NULL	NULL	0	NULL	 interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , cooperative interactions between subunits also affect the voltage dependence of channel opening , and these interactions can be altered by making substitutions at uncharged residues in the S4 region .
	manualset3
87770	5	398742	13	NULL	NULL	0	NULL	substitutions	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , cooperative interactions between subunits also affect the voltage dependence of channel opening , and these interactions can be altered by making substitutions at uncharged residues in the S4 region .
	manualset3
87771	6	398742	13	NULL	NULL	0	NULL	uncharged residues in the S4 region	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	However , cooperative interactions between subunits also affect the voltage dependence of channel opening , and these interactions can be altered by making substitutions at uncharged residues in the S4 region .
	manualset3
87890	1	398743	13	NULL	NULL	0	NULL	clinical course	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( The clinical course of acute brain injuries in deep cranial wounds ) .
	manualset3
87891	2	398743	13	NULL	NULL	0	NULL	acute brain injuries 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( The clinical course of acute brain injuries in deep cranial wounds ) .
	manualset3
87892	3	398743	13	NULL	NULL	0	NULL	cranial wounds	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( The clinical course of acute brain injuries in deep cranial wounds ) .
	manualset3
87893	1	398744	13	NULL	NULL	0	NULL	NO production 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , despite elevated NO production by murine cells , blockage of NO synthesis with the l-arginine analog N-monomethyl-l-arginine only partially rescued chlamydial growth , suggesting the presence of another IFN-gamma-inducible antichlamydial mechanism unique to murine cells .
	manualset3
87894	2	398744	13	NULL	NULL	0	NULL	murine cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , despite elevated NO production by murine cells , blockage of NO synthesis with the l-arginine analog N-monomethyl-l-arginine only partially rescued chlamydial growth , suggesting the presence of another IFN-gamma-inducible antichlamydial mechanism unique to murine cells .
	manualset3
87895	3	398744	13	NULL	NULL	0	NULL	NO synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , despite elevated NO production by murine cells , blockage of NO synthesis with the l-arginine analog N-monomethyl-l-arginine only partially rescued chlamydial growth , suggesting the presence of another IFN-gamma-inducible antichlamydial mechanism unique to murine cells .
	manualset3
87896	4	398744	13	NULL	NULL	NULL	NULL	l-arginine analog N-monomethyl-l-arginine	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , despite elevated NO production by murine cells , blockage of NO synthesis with the l-arginine analog N-monomethyl-l-arginine only partially rescued chlamydial growth , suggesting the presence of another IFN-gamma-inducible antichlamydial mechanism unique to murine cells .
	manualset3
87897	5	398744	13	NULL	NULL	0	NULL	chlamydial growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , despite elevated NO production by murine cells , blockage of NO synthesis with the l-arginine analog N-monomethyl-l-arginine only partially rescued chlamydial growth , suggesting the presence of another IFN-gamma-inducible antichlamydial mechanism unique to murine cells .
	manualset3
87898	6	398744	13	NULL	NULL	0	NULL	IFN-gamma-inducible antichlamydial mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , despite elevated NO production by murine cells , blockage of NO synthesis with the l-arginine analog N-monomethyl-l-arginine only partially rescued chlamydial growth , suggesting the presence of another IFN-gamma-inducible antichlamydial mechanism unique to murine cells .
	manualset3
87899	7	398744	13	NULL	NULL	0	NULL	murine cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , despite elevated NO production by murine cells , blockage of NO synthesis with the l-arginine analog N-monomethyl-l-arginine only partially rescued chlamydial growth , suggesting the presence of another IFN-gamma-inducible antichlamydial mechanism unique to murine cells .
	manualset3
87900	1	398745	13	NULL	NULL	0	NULL	molecular activation mechanism ( s )	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , despite such advances in our understanding of the molecular activation mechanism ( s ) and physiological functions of NDR kinases in yeast and invertebrates , most biological NDR substrates still remain to be identified .
	manualset3
87901	2	398745	13	NULL	NULL	NULL	NULL	physiological functions 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , despite such advances in our understanding of the molecular activation mechanism ( s ) and physiological functions of NDR kinases in yeast and invertebrates , most biological NDR substrates still remain to be identified .
	manualset3
87902	3	398745	13	NULL	NULL	0	NULL	NDR kinases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , despite such advances in our understanding of the molecular activation mechanism ( s ) and physiological functions of NDR kinases in yeast and invertebrates , most biological NDR substrates still remain to be identified .
	manualset3
87903	4	398745	13	NULL	NULL	0	NULL	yeast 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , despite such advances in our understanding of the molecular activation mechanism ( s ) and physiological functions of NDR kinases in yeast and invertebrates , most biological NDR substrates still remain to be identified .
	manualset3
87904	5	398745	13	NULL	NULL	0	NULL	invertebrates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , despite such advances in our understanding of the molecular activation mechanism ( s ) and physiological functions of NDR kinases in yeast and invertebrates , most biological NDR substrates still remain to be identified .
	manualset3
87905	6	398745	13	NULL	NULL	0	NULL	biological NDR substrates	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , despite such advances in our understanding of the molecular activation mechanism ( s ) and physiological functions of NDR kinases in yeast and invertebrates , most biological NDR substrates still remain to be identified .
	manualset3
87906	1	398746	13	NULL	NULL	0	NULL	ligand	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , different ligand specificities of MDC1-FHA have been reported , and no structure is available .
	manualset3
87907	2	398746	13	NULL	NULL	0	NULL	MDC1-FHA 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , different ligand specificities of MDC1-FHA have been reported , and no structure is available .
	manualset3
87908	1	398747	13	NULL	NULL	NULL	NULL	 comparisons	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , direct comparisons have shown that eradication rates achieved by dual therapy are not as high as those achieved by triple therapy .
	manualset3
87909	2	398747	13	NULL	NULL	0	NULL	 eradication rates	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , direct comparisons have shown that eradication rates achieved by dual therapy are not as high as those achieved by triple therapy .
	manualset3
87910	3	398747	13	NULL	NULL	0	NULL	dual therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , direct comparisons have shown that eradication rates achieved by dual therapy are not as high as those achieved by triple therapy .
	manualset3
87911	4	398747	13	NULL	NULL	0	NULL	triple therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , direct comparisons have shown that eradication rates achieved by dual therapy are not as high as those achieved by triple therapy .
	manualset3
87912	1	398748	13	NULL	NULL	NULL	NULL	artifact 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , doubt remains whether this may be an artifact of education bias in the screening tests used .
	manualset3
87913	2	398748	13	NULL	NULL	0	NULL	education bias	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , doubt remains whether this may be an artifact of education bias in the screening tests used .
	manualset3
87914	3	398748	13	NULL	NULL	0	NULL	screening tests	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , doubt remains whether this may be an artifact of education bias in the screening tests used .
	manualset3
88184	4	398748	13	NULL	NULL	0	NULL	doubt	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , doubt remains whether this may be an artifact of education bias in the screening tests used .
	manualset3
87915	1	398749	13	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , doubts can be raised about their differentiation as separate species .
	manualset3
87916	2	398749	13	NULL	NULL	0	NULL	species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , doubts can be raised about their differentiation as separate species .
	manualset3
87917	1	398750	13	NULL	NULL	NULL	NULL	routine drug susceptibility testing	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , due to technical difficulties , routine drug susceptibility testing of Mycobacterium tuberculosis for pyrazinamide is , in many laboratories , not performed .
	manualset3
87918	2	398750	13	NULL	NULL	0	NULL	Mycobacterium tuberculosis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , due to technical difficulties , routine drug susceptibility testing of Mycobacterium tuberculosis for pyrazinamide is , in many laboratories , not performed .
	manualset3
87919	3	398750	13	NULL	NULL	NULL	NULL	pyrazinamide 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , due to technical difficulties , routine drug susceptibility testing of Mycobacterium tuberculosis for pyrazinamide is , in many laboratories , not performed .
	manualset3
87920	4	398750	13	NULL	NULL	0	NULL	laboratories 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	However , due to technical difficulties , routine drug susceptibility testing of Mycobacterium tuberculosis for pyrazinamide is , in many laboratories , not performed .
	manualset3
88185	5	398750	13	NULL	NULL	0	NULL	technical difficulties	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , due to technical difficulties , routine drug susceptibility testing of Mycobacterium tuberculosis for pyrazinamide is , in many laboratories , not performed .
	manualset3
87921	1	398751	13	NULL	NULL	NULL	NULL	early larval life	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , during early larval life , in the prelude to a free-swimming existence , the innervation fields of motorneurons become restricted to a more limited sector of each muscle block , with individual motorneurons reaching predominantly ventral , medial , or dorsal regions .
	manualset3
87922	2	398751	13	NULL	NULL	0	NULL	 free-swimming existence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , during early larval life , in the prelude to a free-swimming existence , the innervation fields of motorneurons become restricted to a more limited sector of each muscle block , with individual motorneurons reaching predominantly ventral , medial , or dorsal regions .
	manualset3
87923	3	398751	13	NULL	NULL	0	NULL	innervation fields 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , during early larval life , in the prelude to a free-swimming existence , the innervation fields of motorneurons become restricted to a more limited sector of each muscle block , with individual motorneurons reaching predominantly ventral , medial , or dorsal regions .
	manualset3
87924	4	398751	13	NULL	NULL	NULL	NULL	motorneurons	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , during early larval life , in the prelude to a free-swimming existence , the innervation fields of motorneurons become restricted to a more limited sector of each muscle block , with individual motorneurons reaching predominantly ventral , medial , or dorsal regions .
	manualset3
87925	5	398751	13	NULL	NULL	NULL	NULL	muscle block	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , during early larval life , in the prelude to a free-swimming existence , the innervation fields of motorneurons become restricted to a more limited sector of each muscle block , with individual motorneurons reaching predominantly ventral , medial , or dorsal regions .
	manualset3
87926	6	398751	13	NULL	NULL	NULL	NULL	motorneurons	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , during early larval life , in the prelude to a free-swimming existence , the innervation fields of motorneurons become restricted to a more limited sector of each muscle block , with individual motorneurons reaching predominantly ventral , medial , or dorsal regions .
	manualset3
87927	7	398751	13	NULL	NULL	0	NULL	ventral regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , during early larval life , in the prelude to a free-swimming existence , the innervation fields of motorneurons become restricted to a more limited sector of each muscle block , with individual motorneurons reaching predominantly ventral , medial , or dorsal regions .
	manualset3
87928	8	398751	13	NULL	NULL	0	NULL	medial regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , during early larval life , in the prelude to a free-swimming existence , the innervation fields of motorneurons become restricted to a more limited sector of each muscle block , with individual motorneurons reaching predominantly ventral , medial , or dorsal regions .
	manualset3
87929	9	398751	13	NULL	NULL	0	NULL	dorsal regions 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , during early larval life , in the prelude to a free-swimming existence , the innervation fields of motorneurons become restricted to a more limited sector of each muscle block , with individual motorneurons reaching predominantly ventral , medial , or dorsal regions .
	manualset3
87930	1	398752	13	NULL	NULL	0	NULL	dust formulations 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , dust formulations are difficult to apply and require specialized equipment .
	manualset3
87931	2	398752	13	NULL	NULL	0	NULL	equipment	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	However , dust formulations are difficult to apply and require specialized equipment .
	manualset3
88186	1	398753	13	NULL	NULL	NULL	NULL	electron pairs	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , electron pairs emitted by the core-resonant channel also share their energy continuously to jointly conserve the energy of the complete process .
	manualset3
89536	2	398753	13	NULL	NULL	0	NULL	core-resonant channel 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	However , electron pairs emitted by the core-resonant channel also share their energy continuously to jointly conserve the energy of the complete process .
	manualset3
89537	3	398753	13	NULL	NULL	0	NULL	energy	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , electron pairs emitted by the core-resonant channel also share their energy continuously to jointly conserve the energy of the complete process .
	manualset3
89538	4	398753	13	NULL	NULL	0	NULL	energy	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , electron pairs emitted by the core-resonant channel also share their energy continuously to jointly conserve the energy of the complete process .
	manualset3
89539	5	398753	13	NULL	NULL	0	NULL	process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , electron pairs emitted by the core-resonant channel also share their energy continuously to jointly conserve the energy of the complete process .
	manualset3
87932	1	398754	13	NULL	NULL	0	NULL	clinical significance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( The clinical significance of findings in microscopic urinalysis ) .
	manualset3
87933	2	398754	13	NULL	NULL	0	NULL	microscopic urinalysis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( The clinical significance of findings in microscopic urinalysis ) .
	manualset3
87934	1	398755	13	NULL	NULL	0	NULL	electrophysiological studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , electrophysiological studies revealed no alteration in the Ca ( 2 + ) current density , the frequency and amplitude of miniature excitatory postsynaptic currents , and the basal synaptic transmission in the mutant hippocampus .
	manualset3
87935	2	398755	13	NULL	NULL	NULL	NULL	Ca ( 2 + ) current density	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , electrophysiological studies revealed no alteration in the Ca ( 2 + ) current density , the frequency and amplitude of miniature excitatory postsynaptic currents , and the basal synaptic transmission in the mutant hippocampus .
	manualset3
87936	3	398755	13	NULL	NULL	0	NULL	frequency 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , electrophysiological studies revealed no alteration in the Ca ( 2 + ) current density , the frequency and amplitude of miniature excitatory postsynaptic currents , and the basal synaptic transmission in the mutant hippocampus .
	manualset3
87937	4	398755	13	NULL	NULL	NULL	NULL	amplitude 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , electrophysiological studies revealed no alteration in the Ca ( 2 + ) current density , the frequency and amplitude of miniature excitatory postsynaptic currents , and the basal synaptic transmission in the mutant hippocampus .
	manualset3
87938	5	398755	13	NULL	NULL	0	NULL	 miniature excitatory postsynaptic currents	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , electrophysiological studies revealed no alteration in the Ca ( 2 + ) current density , the frequency and amplitude of miniature excitatory postsynaptic currents , and the basal synaptic transmission in the mutant hippocampus .
	manualset3
87939	6	398755	13	NULL	NULL	0	NULL	 basal synaptic transmission	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , electrophysiological studies revealed no alteration in the Ca ( 2 + ) current density , the frequency and amplitude of miniature excitatory postsynaptic currents , and the basal synaptic transmission in the mutant hippocampus .
	manualset3
87940	7	398755	13	NULL	NULL	NULL	NULL	mutant hippocampus	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , electrophysiological studies revealed no alteration in the Ca ( 2 + ) current density , the frequency and amplitude of miniature excitatory postsynaptic currents , and the basal synaptic transmission in the mutant hippocampus .
	manualset3
87941	1	398756	13	NULL	NULL	NULL	NULL	 evaluation	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , evaluation of student learning for this kind of simulation focuses mainly on the content and outcome of learning , rather than on the process of learning through student engagement .
	manualset3
87942	2	398756	13	NULL	NULL	NULL	NULL	student 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , evaluation of student learning for this kind of simulation focuses mainly on the content and outcome of learning , rather than on the process of learning through student engagement .
	manualset3
87943	3	398756	13	NULL	NULL	NULL	NULL	learning	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , evaluation of student learning for this kind of simulation focuses mainly on the content and outcome of learning , rather than on the process of learning through student engagement .
	manualset3
87944	4	398756	13	NULL	NULL	NULL	NULL	simulation 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , evaluation of student learning for this kind of simulation focuses mainly on the content and outcome of learning , rather than on the process of learning through student engagement .
	manualset3
87945	5	398756	13	NULL	NULL	0	NULL	learning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , evaluation of student learning for this kind of simulation focuses mainly on the content and outcome of learning , rather than on the process of learning through student engagement .
	manualset3
87946	6	398756	13	NULL	NULL	0	NULL	learning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , evaluation of student learning for this kind of simulation focuses mainly on the content and outcome of learning , rather than on the process of learning through student engagement .
	manualset3
87947	7	398756	13	NULL	NULL	0	NULL	 student	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , evaluation of student learning for this kind of simulation focuses mainly on the content and outcome of learning , rather than on the process of learning through student engagement .
	manualset3
87948	1	398757	13	NULL	NULL	0	NULL	women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , even among women at low risk of recurrence , omitting guideline therapy placed them at elevated risk of recurrence .
	manualset3
87949	2	398757	13	NULL	NULL	0	NULL	low risk of recurrence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , even among women at low risk of recurrence , omitting guideline therapy placed them at elevated risk of recurrence .
	manualset3
87950	3	398757	13	NULL	NULL	0	NULL	omitting guideline therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , even among women at low risk of recurrence , omitting guideline therapy placed them at elevated risk of recurrence .
	manualset3
87951	4	398757	13	NULL	NULL	0	NULL	elevated risk of recurrence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , even among women at low risk of recurrence , omitting guideline therapy placed them at elevated risk of recurrence .
	manualset3
87952	1	398758	13	NULL	NULL	0	NULL	strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , even in strains overproducing L32 mRNA , e.g. from a cDNA copy of the gene , little accumulation of L32 is observed after a brief pulse label .
	manualset3
87953	2	398758	13	NULL	NULL	0	NULL	L32 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	However , even in strains overproducing L32 mRNA , e.g. from a cDNA copy of the gene , little accumulation of L32 is observed after a brief pulse label .
	manualset3
87954	3	398758	13	NULL	NULL	NULL	NULL	 cDNA copy 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , even in strains overproducing L32 mRNA , e.g. from a cDNA copy of the gene , little accumulation of L32 is observed after a brief pulse label .
	manualset3
87955	4	398758	13	NULL	NULL	0	NULL	 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	However , even in strains overproducing L32 mRNA , e.g. from a cDNA copy of the gene , little accumulation of L32 is observed after a brief pulse label .
	manualset3
87956	5	398758	13	NULL	NULL	NULL	NULL	 accumulation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , even in strains overproducing L32 mRNA , e.g. from a cDNA copy of the gene , little accumulation of L32 is observed after a brief pulse label .
	manualset3
87957	6	398758	13	NULL	NULL	NULL	NULL	L32	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , even in strains overproducing L32 mRNA , e.g. from a cDNA copy of the gene , little accumulation of L32 is observed after a brief pulse label .
	manualset3
87958	7	398758	13	NULL	NULL	0	NULL	pulse label 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , even in strains overproducing L32 mRNA , e.g. from a cDNA copy of the gene , little accumulation of L32 is observed after a brief pulse label .
	manualset3
87959	1	398759	13	NULL	NULL	0	NULL	angiographic studies 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , even the most careful angiographic studies do not always totally define the lesion and the surgeon must be prepared to find unexpected vascular relationships at operation .
	manualset3
87960	2	398759	13	NULL	NULL	0	NULL	 lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , even the most careful angiographic studies do not always totally define the lesion and the surgeon must be prepared to find unexpected vascular relationships at operation .
	manualset3
87961	3	398759	13	NULL	NULL	0	NULL	surgeon	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , even the most careful angiographic studies do not always totally define the lesion and the surgeon must be prepared to find unexpected vascular relationships at operation .
	manualset3
87962	4	398759	13	NULL	NULL	0	NULL	relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	However , even the most careful angiographic studies do not always totally define the lesion and the surgeon must be prepared to find unexpected vascular relationships at operation .
	manualset3
87963	5	398759	13	NULL	NULL	0	NULL	operation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , even the most careful angiographic studies do not always totally define the lesion and the surgeon must be prepared to find unexpected vascular relationships at operation .
	manualset3
87964	1	398760	13	NULL	NULL	NULL	NULL	fasting urine calcium excretions 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , fasting urine calcium and magnesium excretions were higher in hypercalciuric calcium stone formers than in healthy control or time-control subjects .
	manualset3
87965	2	398760	13	NULL	NULL	0	NULL	fasting urine magnesium excretions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , fasting urine calcium and magnesium excretions were higher in hypercalciuric calcium stone formers than in healthy control or time-control subjects .
	manualset3
87966	3	398760	13	NULL	NULL	0	NULL	hypercalciuric calcium stone formers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , fasting urine calcium and magnesium excretions were higher in hypercalciuric calcium stone formers than in healthy control or time-control subjects .
	manualset3
87967	4	398760	13	NULL	NULL	0	NULL	healthy control	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , fasting urine calcium and magnesium excretions were higher in hypercalciuric calcium stone formers than in healthy control or time-control subjects .
	manualset3
87968	5	398760	13	NULL	NULL	0	NULL	time-control subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , fasting urine calcium and magnesium excretions were higher in hypercalciuric calcium stone formers than in healthy control or time-control subjects .
	manualset3
87969	1	398761	13	NULL	NULL	0	NULL	XPY	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , feeding XPY alone tended to increase total tract digestibility of organic matter , N , neutral detergent fiber , and acid detergent fiber .
	manualset3
87970	2	398761	13	NULL	NULL	0	NULL	tract digestibility 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , feeding XPY alone tended to increase total tract digestibility of organic matter , N , neutral detergent fiber , and acid detergent fiber .
	manualset3
87971	3	398761	13	NULL	NULL	0	NULL	organic matter	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , feeding XPY alone tended to increase total tract digestibility of organic matter , N , neutral detergent fiber , and acid detergent fiber .
	manualset3
87972	4	398761	13	NULL	NULL	NULL	NULL	N , neutral detergent fiber	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , feeding XPY alone tended to increase total tract digestibility of organic matter , N , neutral detergent fiber , and acid detergent fiber .
	manualset3
87973	5	398761	13	NULL	NULL	NULL	NULL	acid detergent fiber 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , feeding XPY alone tended to increase total tract digestibility of organic matter , N , neutral detergent fiber , and acid detergent fiber .
	manualset3
87974	1	398762	13	NULL	NULL	0	NULL	quantitative assessment measures 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , few , if any , quantitative assessment measures exist ; most descriptions in the literature are qualitative , and this has limited the scope and robustness of research into the problem .
	manualset3
87975	2	398762	13	NULL	NULL	NULL	NULL	descriptions in the literature	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , few , if any , quantitative assessment measures exist ; most descriptions in the literature are qualitative , and this has limited the scope and robustness of research into the problem .
	manualset3
87976	3	398762	13	NULL	NULL	0	NULL	scope	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , few , if any , quantitative assessment measures exist ; most descriptions in the literature are qualitative , and this has limited the scope and robustness of research into the problem .
	manualset3
87977	4	398762	13	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , few , if any , quantitative assessment measures exist ; most descriptions in the literature are qualitative , and this has limited the scope and robustness of research into the problem .
	manualset3
87978	1	398763	13	NULL	NULL	0	NULL	 Analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Analysis of spermatogenesis in senescence-accelerated mice ) .
	manualset3
87979	2	398763	13	NULL	NULL	0	NULL	spermatogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Analysis of spermatogenesis in senescence-accelerated mice ) .
	manualset3
87980	3	398763	13	NULL	NULL	0	NULL	senescence-accelerated mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Analysis of spermatogenesis in senescence-accelerated mice ) .
	manualset3
87981	1	398764	13	NULL	NULL	NULL	NULL	compliance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The compliance of the respiratory system in healthy and respiratory ill newborns after birth and its prognostic value for ventilatory support ( author 's transl ) ) .
	manualset3
87982	2	398764	13	NULL	NULL	0	NULL	respiratory system 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( The compliance of the respiratory system in healthy and respiratory ill newborns after birth and its prognostic value for ventilatory support ( author 's transl ) ) .
	manualset3
87983	3	398764	13	NULL	NULL	0	NULL	 healthy	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( The compliance of the respiratory system in healthy and respiratory ill newborns after birth and its prognostic value for ventilatory support ( author 's transl ) ) .
	manualset3
87984	4	398764	13	NULL	NULL	0	NULL	respiratory ill newborns	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( The compliance of the respiratory system in healthy and respiratory ill newborns after birth and its prognostic value for ventilatory support ( author 's transl ) ) .
	manualset3
87985	5	398764	13	NULL	NULL	NULL	NULL	birth	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The compliance of the respiratory system in healthy and respiratory ill newborns after birth and its prognostic value for ventilatory support ( author 's transl ) ) .
	manualset3
87986	6	398764	13	NULL	NULL	0	NULL	prognostic value	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( The compliance of the respiratory system in healthy and respiratory ill newborns after birth and its prognostic value for ventilatory support ( author 's transl ) ) .
	manualset3
87987	7	398764	13	NULL	NULL	0	NULL	ventilatory support	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( The compliance of the respiratory system in healthy and respiratory ill newborns after birth and its prognostic value for ventilatory support ( author 's transl ) ) .
	manualset3
87988	1	398765	13	NULL	NULL	0	NULL	flavonoids	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , flavonoids with 7-methoxy or 8-hydroxyl groups on the A ring showed only anti-aromatase activity .
	manualset3
87989	2	398765	13	NULL	NULL	0	NULL	7-methoxy or 8-hydroxyl groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , flavonoids with 7-methoxy or 8-hydroxyl groups on the A ring showed only anti-aromatase activity .
	manualset3
87990	3	398765	13	NULL	NULL	0	NULL	anti-aromatase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , flavonoids with 7-methoxy or 8-hydroxyl groups on the A ring showed only anti-aromatase activity .
	manualset3
87991	1	398766	13	NULL	NULL	0	NULL	immunisation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , following immunisation with xenogenic K562 cells , devils did produce cytotoxic responses and antibodies against this foreign tumor cell line .
	manualset3
87992	2	398766	13	NULL	NULL	0	NULL	xenogenic K562 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , following immunisation with xenogenic K562 cells , devils did produce cytotoxic responses and antibodies against this foreign tumor cell line .
	manualset3
87993	3	398766	13	NULL	NULL	0	NULL	devils	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , following immunisation with xenogenic K562 cells , devils did produce cytotoxic responses and antibodies against this foreign tumor cell line .
	manualset3
87994	4	398766	13	NULL	NULL	0	NULL	cytotoxic responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , following immunisation with xenogenic K562 cells , devils did produce cytotoxic responses and antibodies against this foreign tumor cell line .
	manualset3
87995	5	398766	13	NULL	NULL	NULL	NULL	 antibodies 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , following immunisation with xenogenic K562 cells , devils did produce cytotoxic responses and antibodies against this foreign tumor cell line .
	manualset3
87996	6	398766	13	NULL	NULL	0	NULL	foreign tumor cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , following immunisation with xenogenic K562 cells , devils did produce cytotoxic responses and antibodies against this foreign tumor cell line .
	manualset3
87997	1	398767	13	NULL	NULL	0	NULL	mutant of M. fortuitum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , for a mutant of M. fortuitum ( gamma 27 ) with virtually nonexistent beta-lactamase production , the antibiotics still had relatively high MICs ( for instance , benzylpenicillin and cephaloridine had MICs of 64 and 32 micrograms/ml , respectively ) .
	manualset3
87998	2	398767	13	NULL	NULL	0	NULL	gamma 27	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , for a mutant of M. fortuitum ( gamma 27 ) with virtually nonexistent beta-lactamase production , the antibiotics still had relatively high MICs ( for instance , benzylpenicillin and cephaloridine had MICs of 64 and 32 micrograms/ml , respectively ) .
	manualset3
87999	3	398767	13	NULL	NULL	0	NULL	beta-lactamase production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , for a mutant of M. fortuitum ( gamma 27 ) with virtually nonexistent beta-lactamase production , the antibiotics still had relatively high MICs ( for instance , benzylpenicillin and cephaloridine had MICs of 64 and 32 micrograms/ml , respectively ) .
	manualset3
88000	4	398767	13	NULL	NULL	0	NULL	 antibiotics	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , for a mutant of M. fortuitum ( gamma 27 ) with virtually nonexistent beta-lactamase production , the antibiotics still had relatively high MICs ( for instance , benzylpenicillin and cephaloridine had MICs of 64 and 32 micrograms/ml , respectively ) .
	manualset3
88001	5	398767	13	NULL	NULL	NULL	NULL	MICs	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , for a mutant of M. fortuitum ( gamma 27 ) with virtually nonexistent beta-lactamase production , the antibiotics still had relatively high MICs ( for instance , benzylpenicillin and cephaloridine had MICs of 64 and 32 micrograms/ml , respectively ) .
	manualset3
88002	6	398767	13	NULL	NULL	0	NULL	benzylpenicillin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , for a mutant of M. fortuitum ( gamma 27 ) with virtually nonexistent beta-lactamase production , the antibiotics still had relatively high MICs ( for instance , benzylpenicillin and cephaloridine had MICs of 64 and 32 micrograms/ml , respectively ) .
	manualset3
88003	7	398767	13	NULL	NULL	0	NULL	cephaloridine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , for a mutant of M. fortuitum ( gamma 27 ) with virtually nonexistent beta-lactamase production , the antibiotics still had relatively high MICs ( for instance , benzylpenicillin and cephaloridine had MICs of 64 and 32 micrograms/ml , respectively ) .
	manualset3
88004	8	398767	13	NULL	NULL	0	NULL	MICs 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , for a mutant of M. fortuitum ( gamma 27 ) with virtually nonexistent beta-lactamase production , the antibiotics still had relatively high MICs ( for instance , benzylpenicillin and cephaloridine had MICs of 64 and 32 micrograms/ml , respectively ) .
	manualset3
88005	9	398767	13	NULL	NULL	0	NULL	64 micrograms/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , for a mutant of M. fortuitum ( gamma 27 ) with virtually nonexistent beta-lactamase production , the antibiotics still had relatively high MICs ( for instance , benzylpenicillin and cephaloridine had MICs of 64 and 32 micrograms/ml , respectively ) .
	manualset3
88006	10	398767	13	NULL	NULL	NULL	NULL	32 micrograms/ml 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , for a mutant of M. fortuitum ( gamma 27 ) with virtually nonexistent beta-lactamase production , the antibiotics still had relatively high MICs ( for instance , benzylpenicillin and cephaloridine had MICs of 64 and 32 micrograms/ml , respectively ) .
	manualset3
88007	1	398768	13	NULL	NULL	0	NULL	first-generation adolescents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , for first - and second-generation adolescents , participation in extracurricular activities is associated with higher rather than lower odds of violence compared to their non-participating counterparts .
	manualset3
88008	2	398768	13	NULL	NULL	0	NULL	second-generation adolescents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , for first - and second-generation adolescents , participation in extracurricular activities is associated with higher rather than lower odds of violence compared to their non-participating counterparts .
	manualset3
88009	3	398768	13	NULL	NULL	NULL	NULL	extracurricular activities	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , for first - and second-generation adolescents , participation in extracurricular activities is associated with higher rather than lower odds of violence compared to their non-participating counterparts .
	manualset3
88010	4	398768	13	NULL	NULL	NULL	NULL	violence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , for first - and second-generation adolescents , participation in extracurricular activities is associated with higher rather than lower odds of violence compared to their non-participating counterparts .
	manualset3
88011	5	398768	13	NULL	NULL	0	NULL	non-participating counterparts	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , for first - and second-generation adolescents , participation in extracurricular activities is associated with higher rather than lower odds of violence compared to their non-participating counterparts .
	manualset3
88012	1	398769	13	NULL	NULL	0	NULL	loci in LD	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	However , for loci in LD , GIA is often positive , suggesting that assignment can be improved by combining markers into haplotypes .
	manualset3
88013	2	398769	13	NULL	NULL	NULL	NULL	GIA	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , for loci in LD , GIA is often positive , suggesting that assignment can be improved by combining markers into haplotypes .
	manualset3
88014	3	398769	13	NULL	NULL	NULL	NULL	markers	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , for loci in LD , GIA is often positive , suggesting that assignment can be improved by combining markers into haplotypes .
	manualset3
88015	4	398769	13	NULL	NULL	0	NULL	haplotypes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	However , for loci in LD , GIA is often positive , suggesting that assignment can be improved by combining markers into haplotypes .
	manualset3
88016	1	398770	13	NULL	NULL	0	NULL	infectious diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	However , for many infectious diseases T cells are an important part of naturally acquired protective immune responses , and inducing these by vaccination has been the aim of much research .
	manualset3
88017	2	398770	13	NULL	NULL	0	NULL	T cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , for many infectious diseases T cells are an important part of naturally acquired protective immune responses , and inducing these by vaccination has been the aim of much research .
	manualset3
88018	3	398770	13	NULL	NULL	0	NULL	naturally acquired protective immune responses 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , for many infectious diseases T cells are an important part of naturally acquired protective immune responses , and inducing these by vaccination has been the aim of much research .
	manualset3
88019	4	398770	13	NULL	NULL	0	NULL	vaccination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , for many infectious diseases T cells are an important part of naturally acquired protective immune responses , and inducing these by vaccination has been the aim of much research .
	manualset3
88020	5	398770	13	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , for many infectious diseases T cells are an important part of naturally acquired protective immune responses , and inducing these by vaccination has been the aim of much research .
	manualset3
88021	1	398771	13	NULL	NULL	0	NULL	traditional curriculums	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	( The construction of collective portfolios in traditional curriculums : an innovative approach in teaching-learning ) .
	manualset3
88022	2	398771	13	NULL	NULL	NULL	NULL	 innovative approach	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The construction of collective portfolios in traditional curriculums : an innovative approach in teaching-learning ) .
	manualset3
88023	3	398771	13	NULL	NULL	0	NULL	teaching-learning 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( The construction of collective portfolios in traditional curriculums : an innovative approach in teaching-learning ) .
	manualset3
88024	1	398772	13	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , future studies should consider adopting a framework that explicitly accounts for the genealogical effects of population subdivision and empirical sampling schemes .
	manualset3
88025	2	398772	13	NULL	NULL	0	NULL	 framework	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	However , future studies should consider adopting a framework that explicitly accounts for the genealogical effects of population subdivision and empirical sampling schemes .
	manualset3
88026	3	398772	13	NULL	NULL	0	NULL	genealogical effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , future studies should consider adopting a framework that explicitly accounts for the genealogical effects of population subdivision and empirical sampling schemes .
	manualset3
88027	4	398772	13	NULL	NULL	0	NULL	population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , future studies should consider adopting a framework that explicitly accounts for the genealogical effects of population subdivision and empirical sampling schemes .
	manualset3
88028	5	398772	13	NULL	NULL	0	NULL	subdivision	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , future studies should consider adopting a framework that explicitly accounts for the genealogical effects of population subdivision and empirical sampling schemes .
	manualset3
88029	6	398772	13	NULL	NULL	0	NULL	empirical sampling schemes 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , future studies should consider adopting a framework that explicitly accounts for the genealogical effects of population subdivision and empirical sampling schemes .
	manualset3
88030	1	398773	13	NULL	NULL	0	NULL	gibberellin 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , gibberellin regulates expression of GID1 , GA20ox , and GA3ox , and there is also evidence that it regulates DELLA expression .
	manualset3
88031	2	398773	13	NULL	NULL	0	NULL	expression of GID1	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , gibberellin regulates expression of GID1 , GA20ox , and GA3ox , and there is also evidence that it regulates DELLA expression .
	manualset3
88032	3	398773	13	NULL	NULL	0	NULL	expression of GA20ox	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , gibberellin regulates expression of GID1 , GA20ox , and GA3ox , and there is also evidence that it regulates DELLA expression .
	manualset3
88033	4	398773	13	NULL	NULL	0	NULL	expression of GA3ox	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , gibberellin regulates expression of GID1 , GA20ox , and GA3ox , and there is also evidence that it regulates DELLA expression .
	manualset3
88034	5	398773	13	NULL	NULL	0	NULL	DELLA expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , gibberellin regulates expression of GID1 , GA20ox , and GA3ox , and there is also evidence that it regulates DELLA expression .
	manualset3
88035	1	398774	13	NULL	NULL	0	NULL	hemodialysis patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , hemodialysis patients and hemophiliacs were at higher risk of having HCV infection , since the prevalences were , respectively , 35.1 and 42.4 % in comparison with the blood donors ' prevalence ( 1.1 % ) .
	manualset3
88036	2	398774	13	NULL	NULL	0	NULL	 hemophiliacs	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , hemodialysis patients and hemophiliacs were at higher risk of having HCV infection , since the prevalences were , respectively , 35.1 and 42.4 % in comparison with the blood donors ' prevalence ( 1.1 % ) .
	manualset3
88037	3	398774	13	NULL	NULL	0	NULL	risk of having HCV infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , hemodialysis patients and hemophiliacs were at higher risk of having HCV infection , since the prevalences were , respectively , 35.1 and 42.4 % in comparison with the blood donors ' prevalence ( 1.1 % ) .
	manualset3
88038	4	398774	13	NULL	NULL	0	NULL	 35.1 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , hemodialysis patients and hemophiliacs were at higher risk of having HCV infection , since the prevalences were , respectively , 35.1 and 42.4 % in comparison with the blood donors ' prevalence ( 1.1 % ) .
	manualset3
88039	5	398774	13	NULL	NULL	0	NULL	42.4 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , hemodialysis patients and hemophiliacs were at higher risk of having HCV infection , since the prevalences were , respectively , 35.1 and 42.4 % in comparison with the blood donors ' prevalence ( 1.1 % ) .
	manualset3
88040	6	398774	13	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	However , hemodialysis patients and hemophiliacs were at higher risk of having HCV infection , since the prevalences were , respectively , 35.1 and 42.4 % in comparison with the blood donors ' prevalence ( 1.1 % ) .
	manualset3
88041	7	398774	13	NULL	NULL	0	NULL	blood donors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , hemodialysis patients and hemophiliacs were at higher risk of having HCV infection , since the prevalences were , respectively , 35.1 and 42.4 % in comparison with the blood donors ' prevalence ( 1.1 % ) .
	manualset3
88042	8	398774	13	NULL	NULL	0	NULL	prevalence 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , hemodialysis patients and hemophiliacs were at higher risk of having HCV infection , since the prevalences were , respectively , 35.1 and 42.4 % in comparison with the blood donors ' prevalence ( 1.1 % ) .
	manualset3
88043	9	398774	13	NULL	NULL	0	NULL	prevalences	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , hemodialysis patients and hemophiliacs were at higher risk of having HCV infection , since the prevalences were , respectively , 35.1 and 42.4 % in comparison with the blood donors ' prevalence ( 1.1 % ) .
	manualset3
88044	10	398774	13	NULL	NULL	0	NULL	1.1 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , hemodialysis patients and hemophiliacs were at higher risk of having HCV infection , since the prevalences were , respectively , 35.1 and 42.4 % in comparison with the blood donors ' prevalence ( 1.1 % ) .
	manualset3
88045	1	398775	13	NULL	NULL	NULL	NULL	 higher doses of naltrexone	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , higher doses of naltrexone ( 3.0 and 10.0 mg/kg ) increased latencies of both shocked and unshocked mice .
	manualset3
88047	2	398775	13	NULL	NULL	NULL	NULL	3.0 mg/kg	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , higher doses of naltrexone ( 3.0 and 10.0 mg/kg ) increased latencies of both shocked and unshocked mice .
	manualset3
88048	3	398775	13	NULL	NULL	NULL	NULL	10.0 mg/kg	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , higher doses of naltrexone ( 3.0 and 10.0 mg/kg ) increased latencies of both shocked and unshocked mice .
	manualset3
88049	4	398775	13	NULL	NULL	NULL	NULL	shocked  mice	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , higher doses of naltrexone ( 3.0 and 10.0 mg/kg ) increased latencies of both shocked and unshocked mice .
	manualset3
88050	5	398775	13	NULL	NULL	NULL	NULL	unshocked mice	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , higher doses of naltrexone ( 3.0 and 10.0 mg/kg ) increased latencies of both shocked and unshocked mice .
	manualset3
88051	1	398776	13	NULL	NULL	0	NULL	DA neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , how DA neurons encode negative events in the environment is still unclear because some DA neurons appear to be depressed and others excited by aversive stimuli .
	manualset3
88052	2	398776	13	NULL	NULL	NULL	NULL	negative events	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , how DA neurons encode negative events in the environment is still unclear because some DA neurons appear to be depressed and others excited by aversive stimuli .
	manualset3
88053	3	398776	13	NULL	NULL	0	NULL	environment	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , how DA neurons encode negative events in the environment is still unclear because some DA neurons appear to be depressed and others excited by aversive stimuli .
	manualset3
88054	4	398776	13	NULL	NULL	0	NULL	DA neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , how DA neurons encode negative events in the environment is still unclear because some DA neurons appear to be depressed and others excited by aversive stimuli .
	manualset3
88055	5	398776	13	NULL	NULL	NULL	NULL	 aversive stimuli 	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , how DA neurons encode negative events in the environment is still unclear because some DA neurons appear to be depressed and others excited by aversive stimuli .
	manualset3
88056	1	398777	13	NULL	NULL	0	NULL	ice water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , ice water applied to the roots , which reduces root pressure , rapidly diminished exudation rate .
	manualset3
88057	2	398777	13	NULL	NULL	0	NULL	roots 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , ice water applied to the roots , which reduces root pressure , rapidly diminished exudation rate .
	manualset3
88058	3	398777	13	NULL	NULL	0	NULL	root pressure	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , ice water applied to the roots , which reduces root pressure , rapidly diminished exudation rate .
	manualset3
88059	4	398777	13	NULL	NULL	0	NULL	exudation rate	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , ice water applied to the roots , which reduces root pressure , rapidly diminished exudation rate .
	manualset3
88060	1	398778	13	NULL	NULL	0	NULL	intensive therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , if intensive therapy is combined with a hypoglycemia prevention program , the percentage of HbA1c can be maintained below risk values for the onset or progression of complications , and the frequency of hypoglycemia can be kept low .
	manualset3
88061	2	398778	13	NULL	NULL	0	NULL	hypoglycemia prevention program	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , if intensive therapy is combined with a hypoglycemia prevention program , the percentage of HbA1c can be maintained below risk values for the onset or progression of complications , and the frequency of hypoglycemia can be kept low .
	manualset3
88062	3	398778	13	NULL	NULL	0	NULL	 percentage of HbA1c	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , if intensive therapy is combined with a hypoglycemia prevention program , the percentage of HbA1c can be maintained below risk values for the onset or progression of complications , and the frequency of hypoglycemia can be kept low .
	manualset3
88063	4	398778	13	NULL	NULL	0	NULL	risk values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , if intensive therapy is combined with a hypoglycemia prevention program , the percentage of HbA1c can be maintained below risk values for the onset or progression of complications , and the frequency of hypoglycemia can be kept low .
	manualset3
88064	5	398778	13	NULL	NULL	0	NULL	onset or progression of complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , if intensive therapy is combined with a hypoglycemia prevention program , the percentage of HbA1c can be maintained below risk values for the onset or progression of complications , and the frequency of hypoglycemia can be kept low .
	manualset3
88065	6	398778	13	NULL	NULL	0	NULL	frequency of hypoglycemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , if intensive therapy is combined with a hypoglycemia prevention program , the percentage of HbA1c can be maintained below risk values for the onset or progression of complications , and the frequency of hypoglycemia can be kept low .
	manualset3
88066	1	398779	13	NULL	NULL	0	NULL	ocular toxoplasmosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( The cost of ocular toxoplasmosis ) .
	manualset3
88293	2	398779	13	NULL	NULL	0	NULL	cost	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( The cost of ocular toxoplasmosis ) .
	manualset3
88067	1	398780	13	NULL	NULL	0	NULL	70 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in 70 % of asthmatics with BA exacerbation leukocyte sensitivity to CO2 inhibition diminished .
	manualset3
88068	2	398780	13	NULL	NULL	0	NULL	asthmatics	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in 70 % of asthmatics with BA exacerbation leukocyte sensitivity to CO2 inhibition diminished .
	manualset3
88069	3	398780	13	NULL	NULL	0	NULL	BA	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in 70 % of asthmatics with BA exacerbation leukocyte sensitivity to CO2 inhibition diminished .
	manualset3
88070	4	398780	13	NULL	NULL	0	NULL	leukocyte sensitivity to CO2 inhibition 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in 70 % of asthmatics with BA exacerbation leukocyte sensitivity to CO2 inhibition diminished .
	manualset3
88071	1	398781	13	NULL	NULL	0	NULL	 AMPK ( - / - ) MEFs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in AMPK ( - / - ) MEFs transduced with DN AMPK , MMP-9 expression was suppressed .
	manualset3
88072	2	398781	13	NULL	NULL	0	NULL	DN AMPK	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in AMPK ( - / - ) MEFs transduced with DN AMPK , MMP-9 expression was suppressed .
	manualset3
88073	3	398781	13	NULL	NULL	0	NULL	MMP-9 expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in AMPK ( - / - ) MEFs transduced with DN AMPK , MMP-9 expression was suppressed .
	manualset3
88074	1	398782	13	NULL	NULL	0	NULL	RASMC serum	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in RASMC serum stimulated DNA synthesis and further increased the IC50 value for LPS-stimulated inhibition of thymidine incorporation ( 57.3 + / - 7.8 micrograms ml-1 ) .
	manualset3
88075	2	398782	13	NULL	NULL	0	NULL	DNA synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in RASMC serum stimulated DNA synthesis and further increased the IC50 value for LPS-stimulated inhibition of thymidine incorporation ( 57.3 + / - 7.8 micrograms ml-1 ) .
	manualset3
88076	3	398782	13	NULL	NULL	0	NULL	IC50 value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in RASMC serum stimulated DNA synthesis and further increased the IC50 value for LPS-stimulated inhibition of thymidine incorporation ( 57.3 + / - 7.8 micrograms ml-1 ) .
	manualset3
88077	4	398782	13	NULL	NULL	0	NULL	LPS-stimulated inhibition of thymidine incorporation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in RASMC serum stimulated DNA synthesis and further increased the IC50 value for LPS-stimulated inhibition of thymidine incorporation ( 57.3 + / - 7.8 micrograms ml-1 ) .
	manualset3
88078	5	398782	13	NULL	NULL	0	NULL	 57.3 + / - 7.8 micrograms ml-1 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in RASMC serum stimulated DNA synthesis and further increased the IC50 value for LPS-stimulated inhibition of thymidine incorporation ( 57.3 + / - 7.8 micrograms ml-1 ) .
	manualset3
88079	1	398783	13	NULL	NULL	0	NULL	humid atmosphere	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in a humid atmosphere , heat treatment would transform TCP and TTCP into HA by hydrolytic reactions .
	manualset3
88080	2	398783	13	NULL	NULL	0	NULL	heat treatment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in a humid atmosphere , heat treatment would transform TCP and TTCP into HA by hydrolytic reactions .
	manualset3
88081	3	398783	13	NULL	NULL	0	NULL	TCP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in a humid atmosphere , heat treatment would transform TCP and TTCP into HA by hydrolytic reactions .
	manualset3
88082	4	398783	13	NULL	NULL	0	NULL	TTCP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in a humid atmosphere , heat treatment would transform TCP and TTCP into HA by hydrolytic reactions .
	manualset3
88083	5	398783	13	NULL	NULL	0	NULL	HA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in a humid atmosphere , heat treatment would transform TCP and TTCP into HA by hydrolytic reactions .
	manualset3
88084	6	398783	13	NULL	NULL	0	NULL	hydrolytic reactions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in a humid atmosphere , heat treatment would transform TCP and TTCP into HA by hydrolytic reactions .
	manualset3
88085	1	398784	13	NULL	NULL	NULL	NULL	a two-sided clinical scenario	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , in a two-sided clinical scenario ( eg , a trial comparing similar treatments ) the prerandomisation design is potentially highly inefficient ; the refusal rate was much higher for prerandomisation to standard treatment than for conventional two-sided informed consent .
	manualset3
88086	2	398784	13	NULL	NULL	NULL	NULL	a trial comparing similar treatments	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , in a two-sided clinical scenario ( eg , a trial comparing similar treatments ) the prerandomisation design is potentially highly inefficient ; the refusal rate was much higher for prerandomisation to standard treatment than for conventional two-sided informed consent .
	manualset3
88087	3	398784	13	NULL	NULL	0	NULL	prerandomisation design	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in a two-sided clinical scenario ( eg , a trial comparing similar treatments ) the prerandomisation design is potentially highly inefficient ; the refusal rate was much higher for prerandomisation to standard treatment than for conventional two-sided informed consent .
	manualset3
88088	4	398784	13	NULL	NULL	0	NULL	refusal rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in a two-sided clinical scenario ( eg , a trial comparing similar treatments ) the prerandomisation design is potentially highly inefficient ; the refusal rate was much higher for prerandomisation to standard treatment than for conventional two-sided informed consent .
	manualset3
88089	5	398784	13	NULL	NULL	0	NULL	prerandomisation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in a two-sided clinical scenario ( eg , a trial comparing similar treatments ) the prerandomisation design is potentially highly inefficient ; the refusal rate was much higher for prerandomisation to standard treatment than for conventional two-sided informed consent .
	manualset3
88090	6	398784	13	NULL	NULL	0	NULL	standard treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in a two-sided clinical scenario ( eg , a trial comparing similar treatments ) the prerandomisation design is potentially highly inefficient ; the refusal rate was much higher for prerandomisation to standard treatment than for conventional two-sided informed consent .
	manualset3
88091	7	398784	13	NULL	NULL	0	NULL	conventional two-sided informed consent	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in a two-sided clinical scenario ( eg , a trial comparing similar treatments ) the prerandomisation design is potentially highly inefficient ; the refusal rate was much higher for prerandomisation to standard treatment than for conventional two-sided informed consent .
	manualset3
88092	1	398785	13	NULL	NULL	0	NULL	sub-active dose of the selective 5-HT reuptake inhibitor citalopram 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in combination with a sub-active dose of the selective 5-HT reuptake inhibitor citalopram , inducing ~ 50 % 5-HT reuptake inhibition , PNU-282987 has shown marked antidepressant-like effects in the mFST .
	manualset3
88093	2	398785	13	NULL	NULL	0	NULL	~ 50 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in combination with a sub-active dose of the selective 5-HT reuptake inhibitor citalopram , inducing ~ 50 % 5-HT reuptake inhibition , PNU-282987 has shown marked antidepressant-like effects in the mFST .
	manualset3
88094	3	398785	13	NULL	NULL	NULL	NULL	5-HT reuptake inhibition	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , in combination with a sub-active dose of the selective 5-HT reuptake inhibitor citalopram , inducing ~ 50 % 5-HT reuptake inhibition , PNU-282987 has shown marked antidepressant-like effects in the mFST .
	manualset3
88095	4	398785	13	NULL	NULL	0	NULL	 PNU-282987 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in combination with a sub-active dose of the selective 5-HT reuptake inhibitor citalopram , inducing ~ 50 % 5-HT reuptake inhibition , PNU-282987 has shown marked antidepressant-like effects in the mFST .
	manualset3
88096	5	398785	13	NULL	NULL	0	NULL	antidepressant-like effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in combination with a sub-active dose of the selective 5-HT reuptake inhibitor citalopram , inducing ~ 50 % 5-HT reuptake inhibition , PNU-282987 has shown marked antidepressant-like effects in the mFST .
	manualset3
88097	6	398785	13	NULL	NULL	0	NULL	mFST	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in combination with a sub-active dose of the selective 5-HT reuptake inhibitor citalopram , inducing ~ 50 % 5-HT reuptake inhibition , PNU-282987 has shown marked antidepressant-like effects in the mFST .
	manualset3
88098	1	398786	13	NULL	NULL	0	NULL	female rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in intact female rats only MA1 was formed , although the amount of MA , formed in females was much less than in males .
	manualset3
88099	2	398786	13	NULL	NULL	0	NULL	MA1	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in intact female rats only MA1 was formed , although the amount of MA , formed in females was much less than in males .
	manualset3
88100	3	398786	13	NULL	NULL	0	NULL	amount of MA	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in intact female rats only MA1 was formed , although the amount of MA , formed in females was much less than in males .
	manualset3
88101	4	398786	13	NULL	NULL	0	NULL	females	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in intact female rats only MA1 was formed , although the amount of MA , formed in females was much less than in males .
	manualset3
88102	5	398786	13	NULL	NULL	0	NULL	 males	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in intact female rats only MA1 was formed , although the amount of MA , formed in females was much less than in males .
	manualset3
88103	1	398787	13	NULL	NULL	0	NULL	HIV-1	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in many cases , it has been found that HIV-1 can enhance the level of expression and hence the life cycle of other viruses independently of immunosuppression through specific interactions with the viruses .
	manualset3
88104	2	398787	13	NULL	NULL	0	NULL	level of expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in many cases , it has been found that HIV-1 can enhance the level of expression and hence the life cycle of other viruses independently of immunosuppression through specific interactions with the viruses .
	manualset3
88105	3	398787	13	NULL	NULL	NULL	NULL	life cycle 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , in many cases , it has been found that HIV-1 can enhance the level of expression and hence the life cycle of other viruses independently of immunosuppression through specific interactions with the viruses .
	manualset3
88106	4	398787	13	NULL	NULL	0	NULL	viruses 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in many cases , it has been found that HIV-1 can enhance the level of expression and hence the life cycle of other viruses independently of immunosuppression through specific interactions with the viruses .
	manualset3
88107	5	398787	13	NULL	NULL	0	NULL	immunosuppression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in many cases , it has been found that HIV-1 can enhance the level of expression and hence the life cycle of other viruses independently of immunosuppression through specific interactions with the viruses .
	manualset3
88108	6	398787	13	NULL	NULL	0	NULL	interactions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in many cases , it has been found that HIV-1 can enhance the level of expression and hence the life cycle of other viruses independently of immunosuppression through specific interactions with the viruses .
	manualset3
88109	7	398787	13	NULL	NULL	0	NULL	viruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in many cases , it has been found that HIV-1 can enhance the level of expression and hence the life cycle of other viruses independently of immunosuppression through specific interactions with the viruses .
	manualset3
89672	8	398787	13	NULL	NULL	0	NULL	many cases	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in many cases , it has been found that HIV-1 can enhance the level of expression and hence the life cycle of other viruses independently of immunosuppression through specific interactions with the viruses .
	manualset3
88110	1	398788	13	NULL	NULL	0	NULL	occipital structures	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in occipital and occipitotemporal structures , only beta , gamma , and high-gamma amplitudes were robustly strengthened by memory load .
	manualset3
88111	2	398788	13	NULL	NULL	0	NULL	occipitotemporal structures	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in occipital and occipitotemporal structures , only beta , gamma , and high-gamma amplitudes were robustly strengthened by memory load .
	manualset3
88112	3	398788	13	NULL	NULL	NULL	NULL	beta amplitudes	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , in occipital and occipitotemporal structures , only beta , gamma , and high-gamma amplitudes were robustly strengthened by memory load .
	manualset3
88294	4	398788	13	NULL	NULL	0	NULL	gamma amplitudes 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in occipital and occipitotemporal structures , only beta , gamma , and high-gamma amplitudes were robustly strengthened by memory load .
	manualset3
88295	5	398788	13	NULL	NULL	0	NULL	high-gamma amplitudes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in occipital and occipitotemporal structures , only beta , gamma , and high-gamma amplitudes were robustly strengthened by memory load .
	manualset3
88296	6	398788	13	NULL	NULL	0	NULL	memory load	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in occipital and occipitotemporal structures , only beta , gamma , and high-gamma amplitudes were robustly strengthened by memory load .
	manualset3
88113	1	398789	13	NULL	NULL	0	NULL	decision	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in order to take any decision about sports eligibility , sports physicians should perform an initial accurate staging of the bicuspid aortic valve , taking into account hemodynamic factors , aortic complications and associated significant cardiovascular anomalies .
	manualset3
88114	2	398789	13	NULL	NULL	0	NULL	sports physicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in order to take any decision about sports eligibility , sports physicians should perform an initial accurate staging of the bicuspid aortic valve , taking into account hemodynamic factors , aortic complications and associated significant cardiovascular anomalies .
	manualset3
88132	3	398789	13	NULL	NULL	0	NULL	staging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in order to take any decision about sports eligibility , sports physicians should perform an initial accurate staging of the bicuspid aortic valve , taking into account hemodynamic factors , aortic complications and associated significant cardiovascular anomalies .
	manualset3
88133	4	398789	13	NULL	NULL	0	NULL	bicuspid aortic valve	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in order to take any decision about sports eligibility , sports physicians should perform an initial accurate staging of the bicuspid aortic valve , taking into account hemodynamic factors , aortic complications and associated significant cardiovascular anomalies .
	manualset3
88134	5	398789	13	NULL	NULL	0	NULL	hemodynamic factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in order to take any decision about sports eligibility , sports physicians should perform an initial accurate staging of the bicuspid aortic valve , taking into account hemodynamic factors , aortic complications and associated significant cardiovascular anomalies .
	manualset3
88135	6	398789	13	NULL	NULL	0	NULL	aortic complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in order to take any decision about sports eligibility , sports physicians should perform an initial accurate staging of the bicuspid aortic valve , taking into account hemodynamic factors , aortic complications and associated significant cardiovascular anomalies .
	manualset3
88136	7	398789	13	NULL	NULL	0	NULL	cardiovascular anomalies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in order to take any decision about sports eligibility , sports physicians should perform an initial accurate staging of the bicuspid aortic valve , taking into account hemodynamic factors , aortic complications and associated significant cardiovascular anomalies .
	manualset3
88137	1	398790	13	NULL	NULL	0	NULL	B subunit	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in other preparations of the B subunit , there was an additional inhibitory effect due to small contaminations with the A subunit , which caused increases in intracellular cyclic adenosine monophosphate ( cAMP ) levels and concomitant growth inhibition .
	manualset3
88138	2	398790	13	NULL	NULL	NULL	NULL	contaminations 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , in other preparations of the B subunit , there was an additional inhibitory effect due to small contaminations with the A subunit , which caused increases in intracellular cyclic adenosine monophosphate ( cAMP ) levels and concomitant growth inhibition .
	manualset3
88139	3	398790	13	NULL	NULL	0	NULL	A subunit 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in other preparations of the B subunit , there was an additional inhibitory effect due to small contaminations with the A subunit , which caused increases in intracellular cyclic adenosine monophosphate ( cAMP ) levels and concomitant growth inhibition .
	manualset3
88141	5	398790	13	NULL	NULL	0	NULL	growth inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in other preparations of the B subunit , there was an additional inhibitory effect due to small contaminations with the A subunit , which caused increases in intracellular cyclic adenosine monophosphate ( cAMP ) levels and concomitant growth inhibition .
	manualset3
89675	6	398790	13	NULL	NULL	0	NULL	intracellular cyclic adenosine monophosphate ( cAMP ) levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in other preparations of the B subunit , there was an additional inhibitory effect due to small contaminations with the A subunit , which caused increases in intracellular cyclic adenosine monophosphate ( cAMP ) levels and concomitant growth inhibition .
	manualset3
88140	1	398791	13	NULL	NULL	NULL	NULL	 hypercholesterolemia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , in refractory hypercholesterolemia combination therapy may be required .
	manualset3
88142	2	398791	13	NULL	NULL	0	NULL	combination therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in refractory hypercholesterolemia combination therapy may be required .
	manualset3
88143	1	398792	13	NULL	NULL	0	NULL	serum-free conditions 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in serum-free conditions , the rate of enzyme degradation is doubled with no change in the pinocytic rate of the cells .
	manualset3
88144	2	398792	13	NULL	NULL	NULL	NULL	 rate of enzyme degradation 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , in serum-free conditions , the rate of enzyme degradation is doubled with no change in the pinocytic rate of the cells .
	manualset3
88145	3	398792	13	NULL	NULL	0	NULL	pinocytic rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in serum-free conditions , the rate of enzyme degradation is doubled with no change in the pinocytic rate of the cells .
	manualset3
88146	4	398792	13	NULL	NULL	0	NULL	 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in serum-free conditions , the rate of enzyme degradation is doubled with no change in the pinocytic rate of the cells .
	manualset3
88147	1	398793	13	NULL	NULL	0	NULL	translation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in the absence of late translation the L1 pre-mRNA was aberrantly spliced .
	manualset3
88148	2	398793	13	NULL	NULL	0	NULL	L1 pre-mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in the absence of late translation the L1 pre-mRNA was aberrantly spliced .
	manualset3
88149	1	398794	13	NULL	NULL	0	NULL	rose bengal group	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in the illuminated rose bengal group , electrophysiological changes ( inversion of the terminal portion of the T wave and an increase in Q-T interval ) were observed within 11.8 + / - 2.1 seconds ( i.e. , less than 60 beats ) .
	manualset3
88150	2	398794	13	NULL	NULL	NULL	NULL	electrophysiological changes	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , in the illuminated rose bengal group , electrophysiological changes ( inversion of the terminal portion of the T wave and an increase in Q-T interval ) were observed within 11.8 + / - 2.1 seconds ( i.e. , less than 60 beats ) .
	manualset3
88151	3	398794	13	NULL	NULL	NULL	NULL	inversion 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , in the illuminated rose bengal group , electrophysiological changes ( inversion of the terminal portion of the T wave and an increase in Q-T interval ) were observed within 11.8 + / - 2.1 seconds ( i.e. , less than 60 beats ) .
	manualset3
88152	4	398794	13	NULL	NULL	NULL	NULL	Q-T interval 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , in the illuminated rose bengal group , electrophysiological changes ( inversion of the terminal portion of the T wave and an increase in Q-T interval ) were observed within 11.8 + / - 2.1 seconds ( i.e. , less than 60 beats ) .
	manualset3
88153	5	398794	13	NULL	NULL	0	NULL	11.8 + / - 2.1 seconds 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in the illuminated rose bengal group , electrophysiological changes ( inversion of the terminal portion of the T wave and an increase in Q-T interval ) were observed within 11.8 + / - 2.1 seconds ( i.e. , less than 60 beats ) .
	manualset3
88154	6	398794	13	NULL	NULL	0	NULL	less than 60 beats	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in the illuminated rose bengal group , electrophysiological changes ( inversion of the terminal portion of the T wave and an increase in Q-T interval ) were observed within 11.8 + / - 2.1 seconds ( i.e. , less than 60 beats ) .
	manualset3
89540	7	398794	13	NULL	NULL	0	NULL	T wave	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in the illuminated rose bengal group , electrophysiological changes ( inversion of the terminal portion of the T wave and an increase in Q-T interval ) were observed within 11.8 + / - 2.1 seconds ( i.e. , less than 60 beats ) .
	manualset3
88155	1	398795	13	NULL	NULL	NULL	NULL	artificial articular cartilage-PVA-hydrogel 	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The development of a kind of artificial articular cartilage-PVA-hydrogel ) .
	manualset3
88297	2	398795	13	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The development of a kind of artificial articular cartilage-PVA-hydrogel ) .
	manualset3
88156	1	398796	13	NULL	NULL	0	NULL	positive control cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in the positive control cells treated with gliotoxin and PMA ( phorbol 12 myristate-13 acetate ) , a significant increase in apoptotic and necrotic cells was seen .
	manualset3
88157	2	398796	13	NULL	NULL	0	NULL	 gliotoxin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in the positive control cells treated with gliotoxin and PMA ( phorbol 12 myristate-13 acetate ) , a significant increase in apoptotic and necrotic cells was seen .
	manualset3
88158	3	398796	13	NULL	NULL	0	NULL	 PMA ( phorbol 12 myristate-13 acetate )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in the positive control cells treated with gliotoxin and PMA ( phorbol 12 myristate-13 acetate ) , a significant increase in apoptotic and necrotic cells was seen .
	manualset3
88159	4	398796	13	NULL	NULL	0	NULL	apoptotic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in the positive control cells treated with gliotoxin and PMA ( phorbol 12 myristate-13 acetate ) , a significant increase in apoptotic and necrotic cells was seen .
	manualset3
88160	5	398796	13	NULL	NULL	0	NULL	necrotic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in the positive control cells treated with gliotoxin and PMA ( phorbol 12 myristate-13 acetate ) , a significant increase in apoptotic and necrotic cells was seen .
	manualset3
88161	1	398797	13	NULL	NULL	0	NULL	EGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in the presence of EGF , overexpression of ERMBMPs induced remarkable microvillar elongation in A431 cells .
	manualset3
88162	2	398797	13	NULL	NULL	0	NULL	overexpression of ERMBMPs	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in the presence of EGF , overexpression of ERMBMPs induced remarkable microvillar elongation in A431 cells .
	manualset3
88163	3	398797	13	NULL	NULL	0	NULL	microvillar elongation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in the presence of EGF , overexpression of ERMBMPs induced remarkable microvillar elongation in A431 cells .
	manualset3
88164	4	398797	13	NULL	NULL	0	NULL	A431 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in the presence of EGF , overexpression of ERMBMPs induced remarkable microvillar elongation in A431 cells .
	manualset3
88165	1	398798	13	NULL	NULL	NULL	NULL	pressures	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , in the range of pressures over 10 ( -5 ) Torr the measured tritium counting rate was found to be getting smaller than the expected with increase in tritium pressure .
	manualset3
88166	2	398798	13	NULL	NULL	0	NULL	tritium counting rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in the range of pressures over 10 ( -5 ) Torr the measured tritium counting rate was found to be getting smaller than the expected with increase in tritium pressure .
	manualset3
88167	3	398798	13	NULL	NULL	0	NULL	tritium pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in the range of pressures over 10 ( -5 ) Torr the measured tritium counting rate was found to be getting smaller than the expected with increase in tritium pressure .
	manualset3
88298	4	398798	13	NULL	NULL	0	NULL	 10 ( -5 ) Torr	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in the range of pressures over 10 ( -5 ) Torr the measured tritium counting rate was found to be getting smaller than the expected with increase in tritium pressure .
	manualset3
88168	1	398799	13	NULL	NULL	NULL	NULL	research field	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , in the research field , we emphasize the need to look for other methods to improve reverse cholesterol transport , irrespective of HDL-C levels .
	manualset3
88169	2	398799	13	NULL	NULL	NULL	NULL	 methods	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , in the research field , we emphasize the need to look for other methods to improve reverse cholesterol transport , irrespective of HDL-C levels .
	manualset3
88170	3	398799	13	NULL	NULL	NULL	NULL	cholesterol transport	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , in the research field , we emphasize the need to look for other methods to improve reverse cholesterol transport , irrespective of HDL-C levels .
	manualset3
88171	4	398799	13	NULL	NULL	0	NULL	HDL-C levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in the research field , we emphasize the need to look for other methods to improve reverse cholesterol transport , irrespective of HDL-C levels .
	manualset3
88172	1	398800	13	NULL	NULL	0	NULL	new class of agents	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , introduction of the new class of agents that target beta-glucan synthase ( echinocandins ) has invigorated the prospects of combination therapy .
	manualset3
88173	2	398800	13	NULL	NULL	0	NULL	beta-glucan synthase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , introduction of the new class of agents that target beta-glucan synthase ( echinocandins ) has invigorated the prospects of combination therapy .
	manualset3
88174	3	398800	13	NULL	NULL	0	NULL	echinocandins	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , introduction of the new class of agents that target beta-glucan synthase ( echinocandins ) has invigorated the prospects of combination therapy .
	manualset3
88175	4	398800	13	NULL	NULL	0	NULL	combination therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , introduction of the new class of agents that target beta-glucan synthase ( echinocandins ) has invigorated the prospects of combination therapy .
	manualset3
88176	1	398801	13	NULL	NULL	0	NULL	ionophores	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , ionophores ( 200 mM ) in conjunction with TPA ( 20 ng/ml ) induced release of NKCF .
	manualset3
88177	2	398801	13	NULL	NULL	0	NULL	 200 mM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , ionophores ( 200 mM ) in conjunction with TPA ( 20 ng/ml ) induced release of NKCF .
	manualset3
88178	3	398801	13	NULL	NULL	0	NULL	TPA 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , ionophores ( 200 mM ) in conjunction with TPA ( 20 ng/ml ) induced release of NKCF .
	manualset3
88179	4	398801	13	NULL	NULL	0	NULL	20 ng/ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , ionophores ( 200 mM ) in conjunction with TPA ( 20 ng/ml ) induced release of NKCF .
	manualset3
88180	5	398801	13	NULL	NULL	0	NULL	release of NKCF	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , ionophores ( 200 mM ) in conjunction with TPA ( 20 ng/ml ) induced release of NKCF .
	manualset3
88181	1	398802	13	NULL	NULL	NULL	NULL	diagnosis	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The diagnosis of pregnancy ) .
	manualset3
88182	2	398802	13	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( The diagnosis of pregnancy ) .
	manualset3
88183	1	398803	13	NULL	NULL	0	NULL	FDA 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , it is expected that the FDA will soon include cantharidin on its `` Bulk Substances List , '' which would permit physicians or pharmacists to compound cantharidin to be used in the office for individual patients .
	manualset3
88215	2	398803	13	NULL	NULL	0	NULL	cantharidin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , it is expected that the FDA will soon include cantharidin on its `` Bulk Substances List , '' which would permit physicians or pharmacists to compound cantharidin to be used in the office for individual patients .
	manualset3
88216	3	398803	13	NULL	NULL	0	NULL	Bulk Substances List 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , it is expected that the FDA will soon include cantharidin on its `` Bulk Substances List , '' which would permit physicians or pharmacists to compound cantharidin to be used in the office for individual patients .
	manualset3
88217	4	398803	13	NULL	NULL	0	NULL	physicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , it is expected that the FDA will soon include cantharidin on its `` Bulk Substances List , '' which would permit physicians or pharmacists to compound cantharidin to be used in the office for individual patients .
	manualset3
88218	5	398803	13	NULL	NULL	0	NULL	pharmacists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , it is expected that the FDA will soon include cantharidin on its `` Bulk Substances List , '' which would permit physicians or pharmacists to compound cantharidin to be used in the office for individual patients .
	manualset3
88219	6	398803	13	NULL	NULL	0	NULL	cantharidin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , it is expected that the FDA will soon include cantharidin on its `` Bulk Substances List , '' which would permit physicians or pharmacists to compound cantharidin to be used in the office for individual patients .
	manualset3
88220	7	398803	13	NULL	NULL	0	NULL	office	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	However , it is expected that the FDA will soon include cantharidin on its `` Bulk Substances List , '' which would permit physicians or pharmacists to compound cantharidin to be used in the office for individual patients .
	manualset3
88221	8	398803	13	NULL	NULL	0	NULL	individual patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , it is expected that the FDA will soon include cantharidin on its `` Bulk Substances List , '' which would permit physicians or pharmacists to compound cantharidin to be used in the office for individual patients .
	manualset3
88222	1	398804	13	NULL	NULL	0	NULL	PHN 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , it is much less effective against PHN , which occurs more commonly and more severely in older patients .
	manualset3
88223	2	398804	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , it is much less effective against PHN , which occurs more commonly and more severely in older patients .
	manualset3
88224	1	398805	13	NULL	NULL	0	NULL	arginine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	However , it is not known whether such high concentrations of arginine are unique for porcine allantoic fluid or whether they represent an important physiological phenomenon for mammals .
	manualset3
88225	2	398805	13	NULL	NULL	0	NULL	porcine allantoic fluid	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , it is not known whether such high concentrations of arginine are unique for porcine allantoic fluid or whether they represent an important physiological phenomenon for mammals .
	manualset3
88226	3	398805	13	NULL	NULL	0	NULL	physiological phenomenon	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , it is not known whether such high concentrations of arginine are unique for porcine allantoic fluid or whether they represent an important physiological phenomenon for mammals .
	manualset3
88227	4	398805	13	NULL	NULL	0	NULL	mammals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , it is not known whether such high concentrations of arginine are unique for porcine allantoic fluid or whether they represent an important physiological phenomenon for mammals .
	manualset3
88244	5	398805	13	NULL	NULL	0	NULL	concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , it is not known whether such high concentrations of arginine are unique for porcine allantoic fluid or whether they represent an important physiological phenomenon for mammals .
	manualset3
88228	1	398806	13	NULL	NULL	NULL	NULL	training	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , it is unclear how different forms of training affect the response of these hormones .
	manualset3
88229	2	398806	13	NULL	NULL	NULL	NULL	hormones	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , it is unclear how different forms of training affect the response of these hormones .
	manualset3
88230	1	398807	13	NULL	NULL	0	NULL	KIBRA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , it is unclear whether or how KIBRA is connected to the Hippo pathway in mammalian cells .
	manualset3
88231	2	398807	13	NULL	NULL	0	NULL	Hippo pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , it is unclear whether or how KIBRA is connected to the Hippo pathway in mammalian cells .
	manualset3
88232	3	398807	13	NULL	NULL	0	NULL	mammalian cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , it is unclear whether or how KIBRA is connected to the Hippo pathway in mammalian cells .
	manualset3
88233	1	398808	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , it remains unclear whether patients with hematological disorders are at a higher risk of B19 infection .
	manualset3
88234	2	398808	13	NULL	NULL	0	NULL	hematological disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , it remains unclear whether patients with hematological disorders are at a higher risk of B19 infection .
	manualset3
88235	3	398808	13	NULL	NULL	0	NULL	risk of B19 infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , it remains unclear whether patients with hematological disorders are at a higher risk of B19 infection .
	manualset3
88236	1	398809	13	NULL	NULL	0	NULL	zoledronic acid monotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , it was markedly regressed after zoledronic acid monotherapy , and the patient 's symptoms almost disappeared .
	manualset3
88237	2	398809	13	NULL	NULL	0	NULL	patient 's symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , it was markedly regressed after zoledronic acid monotherapy , and the patient 's symptoms almost disappeared .
	manualset3
88238	2	398810	13	NULL	NULL	NULL	NULL	axonal stump	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , it was not the absolute length of the axonal stump that determined the response to transection , but rather its length relative to the lengths of the cell 's other processes .
	manualset3
88239	3	398810	13	NULL	NULL	NULL	NULL	transection	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , it was not the absolute length of the axonal stump that determined the response to transection , but rather its length relative to the lengths of the cell 's other processes .
	manualset3
88240	1	398810	13	NULL	NULL	0	NULL	length	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , it was not the absolute length of the axonal stump that determined the response to transection , but rather its length relative to the lengths of the cell 's other processes .
	manualset3
88241	4	398810	13	NULL	NULL	0	NULL	length 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , it was not the absolute length of the axonal stump that determined the response to transection , but rather its length relative to the lengths of the cell 's other processes .
	manualset3
88242	5	398810	13	NULL	NULL	0	NULL	lengths 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , it was not the absolute length of the axonal stump that determined the response to transection , but rather its length relative to the lengths of the cell 's other processes .
	manualset3
88243	6	398810	13	NULL	NULL	0	NULL	cell 's other processes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	However , it was not the absolute length of the axonal stump that determined the response to transection , but rather its length relative to the lengths of the cell 's other processes .
	manualset3
88245	1	398811	13	NULL	NULL	0	NULL	renin inhibitors	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , large differences between the potencies of renin inhibitors as measured in human and marmoset plasma were observed .
	manualset3
88246	2	398811	13	NULL	NULL	NULL	NULL	human plasma	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , large differences between the potencies of renin inhibitors as measured in human and marmoset plasma were observed .
	manualset3
88247	3	398811	13	NULL	NULL	0	NULL	 marmoset plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , large differences between the potencies of renin inhibitors as measured in human and marmoset plasma were observed .
	manualset3
88248	1	398812	13	NULL	NULL	NULL	NULL	field gradients 	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , later it was recognized that field gradients or inhomogeneous fields were not necessary to separate large DNA fragments , and nowadays , PFGE is generally used to mean pulsed-field gel electrophoresis , i.e. , all kinds of methods involving switching ( pulsing ) of fields to separate large DNAs .
	manualset3
88249	2	398812	13	NULL	NULL	NULL	NULL	inhomogeneous fields	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , later it was recognized that field gradients or inhomogeneous fields were not necessary to separate large DNA fragments , and nowadays , PFGE is generally used to mean pulsed-field gel electrophoresis , i.e. , all kinds of methods involving switching ( pulsing ) of fields to separate large DNAs .
	manualset3
88250	3	398812	13	NULL	NULL	0	NULL	DNA fragments	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	However , later it was recognized that field gradients or inhomogeneous fields were not necessary to separate large DNA fragments , and nowadays , PFGE is generally used to mean pulsed-field gel electrophoresis , i.e. , all kinds of methods involving switching ( pulsing ) of fields to separate large DNAs .
	manualset3
88251	4	398812	13	NULL	NULL	0	NULL	PFGE 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , later it was recognized that field gradients or inhomogeneous fields were not necessary to separate large DNA fragments , and nowadays , PFGE is generally used to mean pulsed-field gel electrophoresis , i.e. , all kinds of methods involving switching ( pulsing ) of fields to separate large DNAs .
	manualset3
88252	5	398812	13	NULL	NULL	0	NULL	pulsed-field gel electrophoresis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , later it was recognized that field gradients or inhomogeneous fields were not necessary to separate large DNA fragments , and nowadays , PFGE is generally used to mean pulsed-field gel electrophoresis , i.e. , all kinds of methods involving switching ( pulsing ) of fields to separate large DNAs .
	manualset3
88253	6	398812	13	NULL	NULL	0	NULL	methods involving switching ( pulsing ) of fields	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , later it was recognized that field gradients or inhomogeneous fields were not necessary to separate large DNA fragments , and nowadays , PFGE is generally used to mean pulsed-field gel electrophoresis , i.e. , all kinds of methods involving switching ( pulsing ) of fields to separate large DNAs .
	manualset3
88254	7	398812	13	NULL	NULL	0	NULL	DNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	However , later it was recognized that field gradients or inhomogeneous fields were not necessary to separate large DNA fragments , and nowadays , PFGE is generally used to mean pulsed-field gel electrophoresis , i.e. , all kinds of methods involving switching ( pulsing ) of fields to separate large DNAs .
	manualset3
88255	1	398813	13	NULL	NULL	0	NULL	learning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , learning to choose advantageously was moderated by sex of participant .
	manualset3
88257	3	398813	13	NULL	NULL	0	NULL	 participant	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , learning to choose advantageously was moderated by sex of participant .
	manualset3
88258	1	398814	13	NULL	NULL	NULL	NULL	 linear acceleration	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , linear acceleration can be received by otolith organ and produce a sensation that is different from that on Earth .
	manualset3
88259	2	398814	13	NULL	NULL	0	NULL	otolith organ	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , linear acceleration can be received by otolith organ and produce a sensation that is different from that on Earth .
	manualset3
88260	3	398814	13	NULL	NULL	0	NULL	sensation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , linear acceleration can be received by otolith organ and produce a sensation that is different from that on Earth .
	manualset3
88261	4	398814	13	NULL	NULL	0	NULL	Earth	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , linear acceleration can be received by otolith organ and produce a sensation that is different from that on Earth .
	manualset3
88262	1	398815	13	NULL	NULL	0	NULL	veins of vascular brain tumors 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( The draining veins of vascular brain tumors in serial angiograms ) .
	manualset3
88263	2	398815	13	NULL	NULL	0	NULL	angiograms	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( The draining veins of vascular brain tumors in serial angiograms ) .
	manualset3
88264	1	398816	13	NULL	NULL	0	NULL	Agrobacterium	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , little is known regarding Agrobacterium persistence in tree species .
	manualset3
88265	2	398816	13	NULL	NULL	0	NULL	persistence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , little is known regarding Agrobacterium persistence in tree species .
	manualset3
88266	3	398816	13	NULL	NULL	0	NULL	 tree species 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , little is known regarding Agrobacterium persistence in tree species .
	manualset3
88267	1	398817	13	NULL	NULL	0	NULL	macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , macrophages of acutely and chronically stressed mice showed inhibition of NO after incubation with MK886 in-vitro .
	manualset3
88268	2	398817	13	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , macrophages of acutely and chronically stressed mice showed inhibition of NO after incubation with MK886 in-vitro .
	manualset3
88269	3	398817	13	NULL	NULL	0	NULL	 inhibition of NO	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , macrophages of acutely and chronically stressed mice showed inhibition of NO after incubation with MK886 in-vitro .
	manualset3
88270	4	398817	13	NULL	NULL	0	NULL	incubation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , macrophages of acutely and chronically stressed mice showed inhibition of NO after incubation with MK886 in-vitro .
	manualset3
88271	5	398817	13	NULL	NULL	0	NULL	MK886	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , macrophages of acutely and chronically stressed mice showed inhibition of NO after incubation with MK886 in-vitro .
	manualset3
88272	1	398818	13	NULL	NULL	0	NULL	male knockout mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , male knockout mice are subfertile and produce sperm with abnormal heads .
	manualset3
88273	2	398818	13	NULL	NULL	0	NULL	subfertile	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , male knockout mice are subfertile and produce sperm with abnormal heads .
	manualset3
88274	3	398818	13	NULL	NULL	0	NULL	 sperm	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , male knockout mice are subfertile and produce sperm with abnormal heads .
	manualset3
88275	4	398818	13	NULL	NULL	0	NULL	abnormal heads	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	However , male knockout mice are subfertile and produce sperm with abnormal heads .
	manualset3
88276	1	398819	13	NULL	NULL	0	NULL	malignant neoplasms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , malignant neoplasms could be differentiated from benign neoplasms in 88 % of the cases .
	manualset3
88277	2	398819	13	NULL	NULL	0	NULL	benign neoplasms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , malignant neoplasms could be differentiated from benign neoplasms in 88 % of the cases .
	manualset3
88278	3	398819	13	NULL	NULL	0	NULL	88 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , malignant neoplasms could be differentiated from benign neoplasms in 88 % of the cases .
	manualset3
88279	4	398819	13	NULL	NULL	0	NULL	 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , malignant neoplasms could be differentiated from benign neoplasms in 88 % of the cases .
	manualset3
88280	1	398820	13	NULL	NULL	0	NULL	disease ( stage IV compared with stage IIIB )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	However , more advanced disease ( stage IV compared with stage IIIB ) was associated with lower SOD activity .
	manualset3
88281	2	398820	13	NULL	NULL	0	NULL	SOD activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , more advanced disease ( stage IV compared with stage IIIB ) was associated with lower SOD activity .
	manualset3
88282	1	398821	13	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , mortality and post-operative stay are not increased .
	manualset3
88283	2	398821	13	NULL	NULL	0	NULL	post-operative stay	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , mortality and post-operative stay are not increased .
	manualset3
88284	1	398822	13	NULL	NULL	0	NULL	12-deoxyphorbol 13-phenylacetate 20-acetate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , neither 12-deoxyphorbol 13-phenylacetate 20-acetate , which selectively activates cPKC-beta , nor ingenol 3 , 20-dibenzoate , which selectively activates nPKC-epsilon , exerted such an effect .
	manualset3
88285	2	398822	13	NULL	NULL	0	NULL	cPKC-beta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , neither 12-deoxyphorbol 13-phenylacetate 20-acetate , which selectively activates cPKC-beta , nor ingenol 3 , 20-dibenzoate , which selectively activates nPKC-epsilon , exerted such an effect .
	manualset3
88286	3	398822	13	NULL	NULL	0	NULL	ingenol 3 , 20-dibenzoate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , neither 12-deoxyphorbol 13-phenylacetate 20-acetate , which selectively activates cPKC-beta , nor ingenol 3 , 20-dibenzoate , which selectively activates nPKC-epsilon , exerted such an effect .
	manualset3
88287	4	398822	13	NULL	NULL	0	NULL	nPKC-epsilon	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , neither 12-deoxyphorbol 13-phenylacetate 20-acetate , which selectively activates cPKC-beta , nor ingenol 3 , 20-dibenzoate , which selectively activates nPKC-epsilon , exerted such an effect .
	manualset3
88288	1	398823	13	NULL	NULL	NULL	NULL	age	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , neither advanced age nor severity of COPD , body mass index , or comorbidity significantly correlated with the total cost .
	manualset3
88289	2	398823	13	NULL	NULL	0	NULL	severity of COPD	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , neither advanced age nor severity of COPD , body mass index , or comorbidity significantly correlated with the total cost .
	manualset3
88290	3	398823	13	NULL	NULL	0	NULL	body mass index	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , neither advanced age nor severity of COPD , body mass index , or comorbidity significantly correlated with the total cost .
	manualset3
88291	4	398823	13	NULL	NULL	0	NULL	comorbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , neither advanced age nor severity of COPD , body mass index , or comorbidity significantly correlated with the total cost .
	manualset3
88292	5	398823	13	NULL	NULL	0	NULL	cost	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , neither advanced age nor severity of COPD , body mass index , or comorbidity significantly correlated with the total cost .
	manualset3
88299	1	398824	13	NULL	NULL	0	NULL	PMB	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	However , neither free PMB nor the PMB-IgG conjugate could protect mice challenged with endotoxin 2 h after administration .
	manualset3
88300	2	398824	13	NULL	NULL	0	NULL	 PMB-IgG conjugate	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , neither free PMB nor the PMB-IgG conjugate could protect mice challenged with endotoxin 2 h after administration .
	manualset3
88301	3	398824	13	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , neither free PMB nor the PMB-IgG conjugate could protect mice challenged with endotoxin 2 h after administration .
	manualset3
88302	4	398824	13	NULL	NULL	0	NULL	 endotoxin 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , neither free PMB nor the PMB-IgG conjugate could protect mice challenged with endotoxin 2 h after administration .
	manualset3
88303	5	398824	13	NULL	NULL	0	NULL	2 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	However , neither free PMB nor the PMB-IgG conjugate could protect mice challenged with endotoxin 2 h after administration .
	manualset3
88304	6	398824	13	NULL	NULL	0	NULL	administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , neither free PMB nor the PMB-IgG conjugate could protect mice challenged with endotoxin 2 h after administration .
	manualset3
88305	1	398825	13	NULL	NULL	0	NULL	2	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , neither of the 2 enriched environments proved consistent superiority or inferiority across all traits .
	manualset3
88306	2	398825	13	NULL	NULL	0	NULL	environments	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , neither of the 2 enriched environments proved consistent superiority or inferiority across all traits .
	manualset3
88307	3	398825	13	NULL	NULL	NULL	NULL	 superiority	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , neither of the 2 enriched environments proved consistent superiority or inferiority across all traits .
	manualset3
88494	4	398825	13	NULL	NULL	0	NULL	 inferiority	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , neither of the 2 enriched environments proved consistent superiority or inferiority across all traits .
	manualset3
88495	5	398825	13	NULL	NULL	0	NULL	traits	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , neither of the 2 enriched environments proved consistent superiority or inferiority across all traits .
	manualset3
88308	1	398826	13	NULL	NULL	0	NULL	 neutralization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , neutralization of TNF-alpha by specific anti-TNF-alpha antibody had no effect on FasL-induced apoptosis .
	manualset3
88309	2	398826	13	NULL	NULL	0	NULL	TNF-alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , neutralization of TNF-alpha by specific anti-TNF-alpha antibody had no effect on FasL-induced apoptosis .
	manualset3
88310	3	398826	13	NULL	NULL	0	NULL	anti-TNF-alpha antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , neutralization of TNF-alpha by specific anti-TNF-alpha antibody had no effect on FasL-induced apoptosis .
	manualset3
88311	4	398826	13	NULL	NULL	0	NULL	FasL-induced apoptosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , neutralization of TNF-alpha by specific anti-TNF-alpha antibody had no effect on FasL-induced apoptosis .
	manualset3
88312	1	398827	13	NULL	NULL	0	NULL	 nitrogenase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , nitrogenase activity under oxic conditions was impaired in strain CSAV135 ( cox3 ) and undetectable in strain CSAV141 ( cox2 cox3 ) .
	manualset3
88313	2	398827	13	NULL	NULL	0	NULL	oxic conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , nitrogenase activity under oxic conditions was impaired in strain CSAV135 ( cox3 ) and undetectable in strain CSAV141 ( cox2 cox3 ) .
	manualset3
88314	3	398827	13	NULL	NULL	0	NULL	strain CSAV135 ( cox3 ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , nitrogenase activity under oxic conditions was impaired in strain CSAV135 ( cox3 ) and undetectable in strain CSAV141 ( cox2 cox3 ) .
	manualset3
88315	4	398827	13	NULL	NULL	0	NULL	strain CSAV141 ( cox2 cox3 ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , nitrogenase activity under oxic conditions was impaired in strain CSAV135 ( cox3 ) and undetectable in strain CSAV141 ( cox2 cox3 ) .
	manualset3
88316	1	398828	13	NULL	NULL	0	NULL	 MVD differences	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , no MVD differences were detected between CLL subgroups subdivided according to the above-mentioned prognostic factors .
	manualset3
88317	2	398828	13	NULL	NULL	0	NULL	CLL subgroups	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	However , no MVD differences were detected between CLL subgroups subdivided according to the above-mentioned prognostic factors .
	manualset3
88318	3	398828	13	NULL	NULL	0	NULL	prognostic factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , no MVD differences were detected between CLL subgroups subdivided according to the above-mentioned prognostic factors .
	manualset3
88319	1	398829	13	NULL	NULL	0	NULL	epithelial defect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , no obvious overlying epithelial defect was detected and an intermittent leakage through micro-perforations in the corneal epithelium was the probable cause of the variable appearance .
	manualset3
88320	2	398829	13	NULL	NULL	0	NULL	leakage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , no obvious overlying epithelial defect was detected and an intermittent leakage through micro-perforations in the corneal epithelium was the probable cause of the variable appearance .
	manualset3
88321	3	398829	13	NULL	NULL	0	NULL	micro-perforations 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , no obvious overlying epithelial defect was detected and an intermittent leakage through micro-perforations in the corneal epithelium was the probable cause of the variable appearance .
	manualset3
88322	4	398829	13	NULL	NULL	0	NULL	corneal epithelium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , no obvious overlying epithelial defect was detected and an intermittent leakage through micro-perforations in the corneal epithelium was the probable cause of the variable appearance .
	manualset3
88323	5	398829	13	NULL	NULL	0	NULL	appearance 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , no obvious overlying epithelial defect was detected and an intermittent leakage through micro-perforations in the corneal epithelium was the probable cause of the variable appearance .
	manualset3
88324	1	398830	13	NULL	NULL	0	NULL	scientific study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , no scientific study has examined the influence of the time of day when strength training is performed on hormonal adaptations .
	manualset3
88325	2	398830	13	NULL	NULL	0	NULL	 influence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , no scientific study has examined the influence of the time of day when strength training is performed on hormonal adaptations .
	manualset3
88326	3	398830	13	NULL	NULL	0	NULL	time of day	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	However , no scientific study has examined the influence of the time of day when strength training is performed on hormonal adaptations .
	manualset3
88327	4	398830	13	NULL	NULL	0	NULL	 strength	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , no scientific study has examined the influence of the time of day when strength training is performed on hormonal adaptations .
	manualset3
88328	5	398830	13	NULL	NULL	0	NULL	training	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , no scientific study has examined the influence of the time of day when strength training is performed on hormonal adaptations .
	manualset3
88329	6	398830	13	NULL	NULL	0	NULL	hormonal adaptations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , no scientific study has examined the influence of the time of day when strength training is performed on hormonal adaptations .
	manualset3
88330	1	398831	13	NULL	NULL	0	NULL	consequences	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The economic consequences of work accidents .
	manualset3
88331	2	398831	13	NULL	NULL	0	NULL	work accidents	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( The economic consequences of work accidents .
	manualset3
88332	1	398832	13	NULL	NULL	0	NULL	( 3H ) leucine incorporation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , no significant difference in ( 3H ) leucine incorporation was observed before or during the initial Ca2 + transport response observed by Halloran and DeLuca , i.e. , at 1.0 , 3.0 , and 6.5 h following an injection of 1 , 25-dihydroxyvitamin D3 .
	manualset3
88333	2	398832	13	NULL	NULL	0	NULL	Ca2 + transport response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , no significant difference in ( 3H ) leucine incorporation was observed before or during the initial Ca2 + transport response observed by Halloran and DeLuca , i.e. , at 1.0 , 3.0 , and 6.5 h following an injection of 1 , 25-dihydroxyvitamin D3 .
	manualset3
88334	3	398832	13	NULL	NULL	0	NULL	Halloran	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	However , no significant difference in ( 3H ) leucine incorporation was observed before or during the initial Ca2 + transport response observed by Halloran and DeLuca , i.e. , at 1.0 , 3.0 , and 6.5 h following an injection of 1 , 25-dihydroxyvitamin D3 .
	manualset3
88335	4	398832	13	NULL	NULL	0	NULL	DeLuca	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	However , no significant difference in ( 3H ) leucine incorporation was observed before or during the initial Ca2 + transport response observed by Halloran and DeLuca , i.e. , at 1.0 , 3.0 , and 6.5 h following an injection of 1 , 25-dihydroxyvitamin D3 .
	manualset3
88336	5	398832	13	NULL	NULL	0	NULL	1.0 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	However , no significant difference in ( 3H ) leucine incorporation was observed before or during the initial Ca2 + transport response observed by Halloran and DeLuca , i.e. , at 1.0 , 3.0 , and 6.5 h following an injection of 1 , 25-dihydroxyvitamin D3 .
	manualset3
88337	6	398832	13	NULL	NULL	0	NULL	3.0 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	However , no significant difference in ( 3H ) leucine incorporation was observed before or during the initial Ca2 + transport response observed by Halloran and DeLuca , i.e. , at 1.0 , 3.0 , and 6.5 h following an injection of 1 , 25-dihydroxyvitamin D3 .
	manualset3
88338	7	398832	13	NULL	NULL	0	NULL	6.5 h 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	However , no significant difference in ( 3H ) leucine incorporation was observed before or during the initial Ca2 + transport response observed by Halloran and DeLuca , i.e. , at 1.0 , 3.0 , and 6.5 h following an injection of 1 , 25-dihydroxyvitamin D3 .
	manualset3
88339	8	398832	13	NULL	NULL	0	NULL	injection 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , no significant difference in ( 3H ) leucine incorporation was observed before or during the initial Ca2 + transport response observed by Halloran and DeLuca , i.e. , at 1.0 , 3.0 , and 6.5 h following an injection of 1 , 25-dihydroxyvitamin D3 .
	manualset3
88340	9	398832	13	NULL	NULL	0	NULL	1 , 25-dihydroxyvitamin D3	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , no significant difference in ( 3H ) leucine incorporation was observed before or during the initial Ca2 + transport response observed by Halloran and DeLuca , i.e. , at 1.0 , 3.0 , and 6.5 h following an injection of 1 , 25-dihydroxyvitamin D3 .
	manualset3
88341	1	398833	13	NULL	NULL	0	NULL	virulence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , no significant virulence differences were observed between wild type , mutant and reconstituted strains in a murine model of pulmonary aspergillosis .
	manualset3
88342	2	398833	13	NULL	NULL	0	NULL	wild type strains 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , no significant virulence differences were observed between wild type , mutant and reconstituted strains in a murine model of pulmonary aspergillosis .
	manualset3
88343	3	398833	13	NULL	NULL	0	NULL	mutant strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , no significant virulence differences were observed between wild type , mutant and reconstituted strains in a murine model of pulmonary aspergillosis .
	manualset3
88344	4	398833	13	NULL	NULL	0	NULL	reconstituted strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , no significant virulence differences were observed between wild type , mutant and reconstituted strains in a murine model of pulmonary aspergillosis .
	manualset3
88345	5	398833	13	NULL	NULL	NULL	NULL	murine model 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , no significant virulence differences were observed between wild type , mutant and reconstituted strains in a murine model of pulmonary aspergillosis .
	manualset3
88346	6	398833	13	NULL	NULL	0	NULL	pulmonary aspergillosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , no significant virulence differences were observed between wild type , mutant and reconstituted strains in a murine model of pulmonary aspergillosis .
	manualset3
88347	1	398834	13	NULL	NULL	0	NULL	32 ( + ) DPZn	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	However , notably 32 ( + ) DPZn achieved remarkably higher ( 1 ) O ( 2 ) - induced cytotoxicity against LLC cells than PIX .
	manualset3
88348	2	398834	13	NULL	NULL	0	NULL	( 1 ) O ( 2 ) 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	However , notably 32 ( + ) DPZn achieved remarkably higher ( 1 ) O ( 2 ) - induced cytotoxicity against LLC cells than PIX .
	manualset3
88350	3	398834	13	NULL	NULL	0	NULL	cytotoxicity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , notably 32 ( + ) DPZn achieved remarkably higher ( 1 ) O ( 2 ) - induced cytotoxicity against LLC cells than PIX .
	manualset3
88351	4	398834	13	NULL	NULL	0	NULL	LLC cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , notably 32 ( + ) DPZn achieved remarkably higher ( 1 ) O ( 2 ) - induced cytotoxicity against LLC cells than PIX .
	manualset3
88352	5	398834	13	NULL	NULL	0	NULL	PIX	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , notably 32 ( + ) DPZn achieved remarkably higher ( 1 ) O ( 2 ) - induced cytotoxicity against LLC cells than PIX .
	manualset3
88365	1	398835	13	NULL	NULL	NULL	NULL	mouse models	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , now that we have mouse or large-animal models for most forms of NCL , we can investigate pathogenesis and compare what happens in the brain in different types of the disease .
	manualset3
88367	2	398835	13	NULL	NULL	NULL	NULL	large-animal models	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , now that we have mouse or large-animal models for most forms of NCL , we can investigate pathogenesis and compare what happens in the brain in different types of the disease .
	manualset3
88371	3	398835	13	NULL	NULL	0	NULL	NCL	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	However , now that we have mouse or large-animal models for most forms of NCL , we can investigate pathogenesis and compare what happens in the brain in different types of the disease .
	manualset3
88372	4	398835	13	NULL	NULL	0	NULL	 pathogenesis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , now that we have mouse or large-animal models for most forms of NCL , we can investigate pathogenesis and compare what happens in the brain in different types of the disease .
	manualset3
88373	5	398835	13	NULL	NULL	0	NULL	brain 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , now that we have mouse or large-animal models for most forms of NCL , we can investigate pathogenesis and compare what happens in the brain in different types of the disease .
	manualset3
88379	6	398835	13	NULL	NULL	0	NULL	disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	However , now that we have mouse or large-animal models for most forms of NCL , we can investigate pathogenesis and compare what happens in the brain in different types of the disease .
	manualset3
88384	1	398836	13	NULL	NULL	0	NULL	 biofilm bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , on suspension of the biofilm bacteria , glycocalyx-mediated resistance was lost .
	manualset3
88385	2	398836	13	NULL	NULL	0	NULL	glycocalyx-mediated resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , on suspension of the biofilm bacteria , glycocalyx-mediated resistance was lost .
	manualset3
88386	3	398836	13	NULL	NULL	0	NULL	 suspension	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	However , on suspension of the biofilm bacteria , glycocalyx-mediated resistance was lost .
	manualset3
88388	1	398837	13	NULL	NULL	0	NULL	mind 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , one should been in mind that systemic heparinization itself carries a potential risk of hemorrhage .
	manualset3
88389	2	398837	13	NULL	NULL	0	NULL	heparinization 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , one should been in mind that systemic heparinization itself carries a potential risk of hemorrhage .
	manualset3
88390	3	398837	13	NULL	NULL	0	NULL	 risk of hemorrhage 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , one should been in mind that systemic heparinization itself carries a potential risk of hemorrhage .
	manualset3
88391	1	398838	13	NULL	NULL	0	NULL	 minority	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , only a minority of familial gastric cancers can be accounted for by CDH1 mutations .
	manualset3
88392	2	398838	13	NULL	NULL	0	NULL	familial gastric cancers	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	However , only a minority of familial gastric cancers can be accounted for by CDH1 mutations .
	manualset3
88393	3	398838	13	NULL	NULL	0	NULL	CDH1 mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , only a minority of familial gastric cancers can be accounted for by CDH1 mutations .
	manualset3
88394	1	398839	13	NULL	NULL	NULL	NULL	small fraction ( 0.07-0 .32 % )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , only a small fraction ( 0.07-0 .32 % ) of the TFIIIB70 from these sources results in the synthesis of full-length RNA .
	manualset3
88397	2	398839	13	NULL	NULL	0	NULL	TFIIIB70	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , only a small fraction ( 0.07-0 .32 % ) of the TFIIIB70 from these sources results in the synthesis of full-length RNA .
	manualset3
88399	3	398839	13	NULL	NULL	0	NULL	synthesis of full-length RNA	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , only a small fraction ( 0.07-0 .32 % ) of the TFIIIB70 from these sources results in the synthesis of full-length RNA .
	manualset3
88423	1	398840	13	NULL	NULL	0	NULL	adrenoblockaders	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effect of adrenoblockaders on the rate of H3-catecholamine synthesis and uptake in the rat seminal duct ) .
	manualset3
88424	2	398840	13	NULL	NULL	0	NULL	rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effect of adrenoblockaders on the rate of H3-catecholamine synthesis and uptake in the rat seminal duct ) .
	manualset3
88425	3	398840	13	NULL	NULL	0	NULL	H3-catecholamine synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effect of adrenoblockaders on the rate of H3-catecholamine synthesis and uptake in the rat seminal duct ) .
	manualset3
88426	4	398840	13	NULL	NULL	0	NULL	uptake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effect of adrenoblockaders on the rate of H3-catecholamine synthesis and uptake in the rat seminal duct ) .
	manualset3
88427	5	398840	13	NULL	NULL	0	NULL	rat seminal duct 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effect of adrenoblockaders on the rate of H3-catecholamine synthesis and uptake in the rat seminal duct ) .
	manualset3
88428	1	398841	13	NULL	NULL	0	NULL	 works 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , only few works focus their attention on its seeds , which constitute a major byproduct of the tomato processing industry .
	manualset3
88430	3	398841	13	NULL	NULL	0	NULL	attention	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , only few works focus their attention on its seeds , which constitute a major byproduct of the tomato processing industry .
	manualset3
88431	4	398841	13	NULL	NULL	0	NULL	seeds	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , only few works focus their attention on its seeds , which constitute a major byproduct of the tomato processing industry .
	manualset3
88433	5	398841	13	NULL	NULL	0	NULL	tomato processing industry	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	However , only few works focus their attention on its seeds , which constitute a major byproduct of the tomato processing industry .
	manualset3
88434	1	398842	13	NULL	NULL	0	NULL	JNK1 isoform 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , only the JNK1 isoform was phosphorylated and , as determined in single knock-out mice , was necessary for Mkp1 induction by M-CSF or LPS .
	manualset3
88435	2	398842	13	NULL	NULL	0	NULL	single knock-out mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , only the JNK1 isoform was phosphorylated and , as determined in single knock-out mice , was necessary for Mkp1 induction by M-CSF or LPS .
	manualset3
88436	3	398842	13	NULL	NULL	0	NULL	Mkp1 induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , only the JNK1 isoform was phosphorylated and , as determined in single knock-out mice , was necessary for Mkp1 induction by M-CSF or LPS .
	manualset3
88437	4	398842	13	NULL	NULL	0	NULL	M-CSF 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , only the JNK1 isoform was phosphorylated and , as determined in single knock-out mice , was necessary for Mkp1 induction by M-CSF or LPS .
	manualset3
88441	5	398842	13	NULL	NULL	0	NULL	 LPS	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , only the JNK1 isoform was phosphorylated and , as determined in single knock-out mice , was necessary for Mkp1 induction by M-CSF or LPS .
	manualset3
88445	1	398843	13	NULL	NULL	0	NULL	mutated peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	However , only the mutated peptide could induce specific CTL expansion from PBL .
	manualset3
88446	2	398843	13	NULL	NULL	0	NULL	CTL expansion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , only the mutated peptide could induce specific CTL expansion from PBL .
	manualset3
88447	3	398843	13	NULL	NULL	0	NULL	PBL	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , only the mutated peptide could induce specific CTL expansion from PBL .
	manualset3
88448	1	398844	13	NULL	NULL	0	NULL	three-quarters 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , only three-quarters of all strokes can be attributable to known causal risk factors .
	manualset3
88449	2	398844	13	NULL	NULL	0	NULL	strokes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , only three-quarters of all strokes can be attributable to known causal risk factors .
	manualset3
88450	3	398844	13	NULL	NULL	0	NULL	risk factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , only three-quarters of all strokes can be attributable to known causal risk factors .
	manualset3
88451	1	398845	13	NULL	NULL	0	NULL	peritoneal exudate cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , peritoneal exudate cells continued to respond to exogenous beta carotene in vitro to produce additional cytotoxic materials .
	manualset3
88452	2	398845	13	NULL	NULL	0	NULL	beta carotene 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , peritoneal exudate cells continued to respond to exogenous beta carotene in vitro to produce additional cytotoxic materials .
	manualset3
88453	3	398845	13	NULL	NULL	0	NULL	cytotoxic materials	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , peritoneal exudate cells continued to respond to exogenous beta carotene in vitro to produce additional cytotoxic materials .
	manualset3
88454	1	398846	13	NULL	NULL	0	NULL	 phylogenetic analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , phylogenetic analysis of rpoD gene sequences showed that strain M1 ( T ) exhibited high sequence similarity only with respect to Pseudomonas psycrophila ( 97.42 % ) and P. fragi ( 96.40 % ) and DNA-DNA hybridization experiments between the Antarctic isolate M1 ( T ) and the type strains of these two closely related species revealed relatedness values of 58 and 57 % , respectively .
	manualset3
88455	2	398846	13	NULL	NULL	0	NULL	 rpoD gene sequences 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	However , phylogenetic analysis of rpoD gene sequences showed that strain M1 ( T ) exhibited high sequence similarity only with respect to Pseudomonas psycrophila ( 97.42 % ) and P. fragi ( 96.40 % ) and DNA-DNA hybridization experiments between the Antarctic isolate M1 ( T ) and the type strains of these two closely related species revealed relatedness values of 58 and 57 % , respectively .
	manualset3
88456	3	398846	13	NULL	NULL	0	NULL	strain M1 ( T )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , phylogenetic analysis of rpoD gene sequences showed that strain M1 ( T ) exhibited high sequence similarity only with respect to Pseudomonas psycrophila ( 97.42 % ) and P. fragi ( 96.40 % ) and DNA-DNA hybridization experiments between the Antarctic isolate M1 ( T ) and the type strains of these two closely related species revealed relatedness values of 58 and 57 % , respectively .
	manualset3
88457	4	398846	13	NULL	NULL	NULL	NULL	sequence similarity	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , phylogenetic analysis of rpoD gene sequences showed that strain M1 ( T ) exhibited high sequence similarity only with respect to Pseudomonas psycrophila ( 97.42 % ) and P. fragi ( 96.40 % ) and DNA-DNA hybridization experiments between the Antarctic isolate M1 ( T ) and the type strains of these two closely related species revealed relatedness values of 58 and 57 % , respectively .
	manualset3
88478	5	398846	13	NULL	NULL	0	NULL	Pseudomonas psycrophila	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , phylogenetic analysis of rpoD gene sequences showed that strain M1 ( T ) exhibited high sequence similarity only with respect to Pseudomonas psycrophila ( 97.42 % ) and P. fragi ( 96.40 % ) and DNA-DNA hybridization experiments between the Antarctic isolate M1 ( T ) and the type strains of these two closely related species revealed relatedness values of 58 and 57 % , respectively .
	manualset3
88479	6	398846	13	NULL	NULL	0	NULL	97.42 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , phylogenetic analysis of rpoD gene sequences showed that strain M1 ( T ) exhibited high sequence similarity only with respect to Pseudomonas psycrophila ( 97.42 % ) and P. fragi ( 96.40 % ) and DNA-DNA hybridization experiments between the Antarctic isolate M1 ( T ) and the type strains of these two closely related species revealed relatedness values of 58 and 57 % , respectively .
	manualset3
88480	7	398846	13	NULL	NULL	0	NULL	P. fragi	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , phylogenetic analysis of rpoD gene sequences showed that strain M1 ( T ) exhibited high sequence similarity only with respect to Pseudomonas psycrophila ( 97.42 % ) and P. fragi ( 96.40 % ) and DNA-DNA hybridization experiments between the Antarctic isolate M1 ( T ) and the type strains of these two closely related species revealed relatedness values of 58 and 57 % , respectively .
	manualset3
88481	8	398846	13	NULL	NULL	0	NULL	96.40 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , phylogenetic analysis of rpoD gene sequences showed that strain M1 ( T ) exhibited high sequence similarity only with respect to Pseudomonas psycrophila ( 97.42 % ) and P. fragi ( 96.40 % ) and DNA-DNA hybridization experiments between the Antarctic isolate M1 ( T ) and the type strains of these two closely related species revealed relatedness values of 58 and 57 % , respectively .
	manualset3
88482	9	398846	13	NULL	NULL	0	NULL	 DNA-DNA hybridization experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , phylogenetic analysis of rpoD gene sequences showed that strain M1 ( T ) exhibited high sequence similarity only with respect to Pseudomonas psycrophila ( 97.42 % ) and P. fragi ( 96.40 % ) and DNA-DNA hybridization experiments between the Antarctic isolate M1 ( T ) and the type strains of these two closely related species revealed relatedness values of 58 and 57 % , respectively .
	manualset3
88484	10	398846	13	NULL	NULL	0	NULL	Antarctic isolate M1 ( T ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , phylogenetic analysis of rpoD gene sequences showed that strain M1 ( T ) exhibited high sequence similarity only with respect to Pseudomonas psycrophila ( 97.42 % ) and P. fragi ( 96.40 % ) and DNA-DNA hybridization experiments between the Antarctic isolate M1 ( T ) and the type strains of these two closely related species revealed relatedness values of 58 and 57 % , respectively .
	manualset3
88485	11	398846	13	NULL	NULL	0	NULL	strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , phylogenetic analysis of rpoD gene sequences showed that strain M1 ( T ) exhibited high sequence similarity only with respect to Pseudomonas psycrophila ( 97.42 % ) and P. fragi ( 96.40 % ) and DNA-DNA hybridization experiments between the Antarctic isolate M1 ( T ) and the type strains of these two closely related species revealed relatedness values of 58 and 57 % , respectively .
	manualset3
88486	12	398846	13	NULL	NULL	NULL	NULL	species	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , phylogenetic analysis of rpoD gene sequences showed that strain M1 ( T ) exhibited high sequence similarity only with respect to Pseudomonas psycrophila ( 97.42 % ) and P. fragi ( 96.40 % ) and DNA-DNA hybridization experiments between the Antarctic isolate M1 ( T ) and the type strains of these two closely related species revealed relatedness values of 58 and 57 % , respectively .
	manualset3
88487	13	398846	13	NULL	NULL	0	NULL	 relatedness values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , phylogenetic analysis of rpoD gene sequences showed that strain M1 ( T ) exhibited high sequence similarity only with respect to Pseudomonas psycrophila ( 97.42 % ) and P. fragi ( 96.40 % ) and DNA-DNA hybridization experiments between the Antarctic isolate M1 ( T ) and the type strains of these two closely related species revealed relatedness values of 58 and 57 % , respectively .
	manualset3
88488	14	398846	13	NULL	NULL	0	NULL	58 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , phylogenetic analysis of rpoD gene sequences showed that strain M1 ( T ) exhibited high sequence similarity only with respect to Pseudomonas psycrophila ( 97.42 % ) and P. fragi ( 96.40 % ) and DNA-DNA hybridization experiments between the Antarctic isolate M1 ( T ) and the type strains of these two closely related species revealed relatedness values of 58 and 57 % , respectively .
	manualset3
88489	15	398846	13	NULL	NULL	0	NULL	57 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , phylogenetic analysis of rpoD gene sequences showed that strain M1 ( T ) exhibited high sequence similarity only with respect to Pseudomonas psycrophila ( 97.42 % ) and P. fragi ( 96.40 % ) and DNA-DNA hybridization experiments between the Antarctic isolate M1 ( T ) and the type strains of these two closely related species revealed relatedness values of 58 and 57 % , respectively .
	manualset3
88490	1	398847	13	NULL	NULL	0	NULL	physiologic tissue oxygenation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , physiologic tissue oxygenation on its own is not enough to prevent toxicity after perfusion .
	manualset3
88491	2	398847	13	NULL	NULL	0	NULL	toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , physiologic tissue oxygenation on its own is not enough to prevent toxicity after perfusion .
	manualset3
88496	3	398847	13	NULL	NULL	0	NULL	perfusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , physiologic tissue oxygenation on its own is not enough to prevent toxicity after perfusion .
	manualset3
88497	1	398848	13	NULL	NULL	0	NULL	 plasma total cholesterol 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , plasma total cholesterol and HDL-cholesterol levels were significantly increased and plasma triglyceride levels were slightly decreased in the pioglitazone + NO-1886 group , compared with the values in the pioglitazone-alone group .
	manualset3
88499	2	398848	13	NULL	NULL	0	NULL	 HDL-cholesterol levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , plasma total cholesterol and HDL-cholesterol levels were significantly increased and plasma triglyceride levels were slightly decreased in the pioglitazone + NO-1886 group , compared with the values in the pioglitazone-alone group .
	manualset3
88501	3	398848	13	NULL	NULL	0	NULL	plasma triglyceride levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , plasma total cholesterol and HDL-cholesterol levels were significantly increased and plasma triglyceride levels were slightly decreased in the pioglitazone + NO-1886 group , compared with the values in the pioglitazone-alone group .
	manualset3
88504	5	398848	13	NULL	NULL	0	NULL	values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , plasma total cholesterol and HDL-cholesterol levels were significantly increased and plasma triglyceride levels were slightly decreased in the pioglitazone + NO-1886 group , compared with the values in the pioglitazone-alone group .
	manualset3
88505	6	398848	13	NULL	NULL	NULL	NULL	pioglitazone-alone group	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , plasma total cholesterol and HDL-cholesterol levels were significantly increased and plasma triglyceride levels were slightly decreased in the pioglitazone + NO-1886 group , compared with the values in the pioglitazone-alone group .
	manualset3
91081	7	398848	13	NULL	NULL	0	NULL	 pioglitazone + NO-1886 group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , plasma total cholesterol and HDL-cholesterol levels were significantly increased and plasma triglyceride levels were slightly decreased in the pioglitazone + NO-1886 group , compared with the values in the pioglitazone-alone group .
	manualset3
88503	1	398849	13	NULL	NULL	NULL	NULL	 pretreatment	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , pretreatment with PD98059 had no effect on EPAS1 phosphorylation during hypoxia , suggesting that MAPK targets other proteins that are critical for the trans-activation of EPAS1 .
	manualset3
88511	2	398849	13	NULL	NULL	0	NULL	PD98059	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , pretreatment with PD98059 had no effect on EPAS1 phosphorylation during hypoxia , suggesting that MAPK targets other proteins that are critical for the trans-activation of EPAS1 .
	manualset3
88512	3	398849	13	NULL	NULL	0	NULL	EPAS1 phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , pretreatment with PD98059 had no effect on EPAS1 phosphorylation during hypoxia , suggesting that MAPK targets other proteins that are critical for the trans-activation of EPAS1 .
	manualset3
88514	4	398849	13	NULL	NULL	0	NULL	hypoxia	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , pretreatment with PD98059 had no effect on EPAS1 phosphorylation during hypoxia , suggesting that MAPK targets other proteins that are critical for the trans-activation of EPAS1 .
	manualset3
88516	5	398849	13	NULL	NULL	0	NULL	MAPK targets	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , pretreatment with PD98059 had no effect on EPAS1 phosphorylation during hypoxia , suggesting that MAPK targets other proteins that are critical for the trans-activation of EPAS1 .
	manualset3
88517	6	398849	13	NULL	NULL	NULL	NULL	 proteins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , pretreatment with PD98059 had no effect on EPAS1 phosphorylation during hypoxia , suggesting that MAPK targets other proteins that are critical for the trans-activation of EPAS1 .
	manualset3
88519	7	398849	13	NULL	NULL	0	NULL	trans-activation of EPAS1	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , pretreatment with PD98059 had no effect on EPAS1 phosphorylation during hypoxia , suggesting that MAPK targets other proteins that are critical for the trans-activation of EPAS1 .
	manualset3
88523	1	398850	13	NULL	NULL	0	NULL	all-trans retinoid acid	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effect of all-trans retinoid acid and sodium selenite ( Na2SeO3 ) on VEGF and its receptor expression in HL-60 cells ) .
	manualset3
88524	2	398850	13	NULL	NULL	0	NULL	sodium selenite ( Na2SeO3 ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effect of all-trans retinoid acid and sodium selenite ( Na2SeO3 ) on VEGF and its receptor expression in HL-60 cells ) .
	manualset3
88526	3	398850	13	NULL	NULL	0	NULL	VEGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effect of all-trans retinoid acid and sodium selenite ( Na2SeO3 ) on VEGF and its receptor expression in HL-60 cells ) .
	manualset3
88528	4	398850	13	NULL	NULL	0	NULL	receptor expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effect of all-trans retinoid acid and sodium selenite ( Na2SeO3 ) on VEGF and its receptor expression in HL-60 cells ) .
	manualset3
88529	5	398850	13	NULL	NULL	0	NULL	HL-60 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effect of all-trans retinoid acid and sodium selenite ( Na2SeO3 ) on VEGF and its receptor expression in HL-60 cells ) .
	manualset3
88542	1	398851	13	NULL	NULL	0	NULL	research 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , previous research did not test whether motion sickness increases anticipatory nausea only by increasing the base rate of posttreatment nausea and vomiting ( which has traditionally served as the unconditioned stimulus in the conditioning model for anticipatory nausea ) or , alternatively , whether motion sickness might facilitate the association of external stimuli to posttreatment nausea and vomiting .
	manualset3
88544	2	398851	13	NULL	NULL	0	NULL	motion sickness 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , previous research did not test whether motion sickness increases anticipatory nausea only by increasing the base rate of posttreatment nausea and vomiting ( which has traditionally served as the unconditioned stimulus in the conditioning model for anticipatory nausea ) or , alternatively , whether motion sickness might facilitate the association of external stimuli to posttreatment nausea and vomiting .
	manualset3
88546	3	398851	13	NULL	NULL	NULL	NULL	anticipatory nausea 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , previous research did not test whether motion sickness increases anticipatory nausea only by increasing the base rate of posttreatment nausea and vomiting ( which has traditionally served as the unconditioned stimulus in the conditioning model for anticipatory nausea ) or , alternatively , whether motion sickness might facilitate the association of external stimuli to posttreatment nausea and vomiting .
	manualset3
88548	4	398851	13	NULL	NULL	0	NULL	rate of posttreatment nausea 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , previous research did not test whether motion sickness increases anticipatory nausea only by increasing the base rate of posttreatment nausea and vomiting ( which has traditionally served as the unconditioned stimulus in the conditioning model for anticipatory nausea ) or , alternatively , whether motion sickness might facilitate the association of external stimuli to posttreatment nausea and vomiting .
	manualset3
88549	5	398851	13	NULL	NULL	0	NULL	vomiting	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , previous research did not test whether motion sickness increases anticipatory nausea only by increasing the base rate of posttreatment nausea and vomiting ( which has traditionally served as the unconditioned stimulus in the conditioning model for anticipatory nausea ) or , alternatively , whether motion sickness might facilitate the association of external stimuli to posttreatment nausea and vomiting .
	manualset3
88550	6	398851	13	NULL	NULL	0	NULL	 stimulus	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , previous research did not test whether motion sickness increases anticipatory nausea only by increasing the base rate of posttreatment nausea and vomiting ( which has traditionally served as the unconditioned stimulus in the conditioning model for anticipatory nausea ) or , alternatively , whether motion sickness might facilitate the association of external stimuli to posttreatment nausea and vomiting .
	manualset3
88552	7	398851	13	NULL	NULL	NULL	NULL	conditioning model	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , previous research did not test whether motion sickness increases anticipatory nausea only by increasing the base rate of posttreatment nausea and vomiting ( which has traditionally served as the unconditioned stimulus in the conditioning model for anticipatory nausea ) or , alternatively , whether motion sickness might facilitate the association of external stimuli to posttreatment nausea and vomiting .
	manualset3
88553	8	398851	13	NULL	NULL	0	NULL	anticipatory nausea 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , previous research did not test whether motion sickness increases anticipatory nausea only by increasing the base rate of posttreatment nausea and vomiting ( which has traditionally served as the unconditioned stimulus in the conditioning model for anticipatory nausea ) or , alternatively , whether motion sickness might facilitate the association of external stimuli to posttreatment nausea and vomiting .
	manualset3
88554	9	398851	13	NULL	NULL	0	NULL	motion sickness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , previous research did not test whether motion sickness increases anticipatory nausea only by increasing the base rate of posttreatment nausea and vomiting ( which has traditionally served as the unconditioned stimulus in the conditioning model for anticipatory nausea ) or , alternatively , whether motion sickness might facilitate the association of external stimuli to posttreatment nausea and vomiting .
	manualset3
88555	10	398851	13	NULL	NULL	0	NULL	stimuli	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , previous research did not test whether motion sickness increases anticipatory nausea only by increasing the base rate of posttreatment nausea and vomiting ( which has traditionally served as the unconditioned stimulus in the conditioning model for anticipatory nausea ) or , alternatively , whether motion sickness might facilitate the association of external stimuli to posttreatment nausea and vomiting .
	manualset3
88556	11	398851	13	NULL	NULL	0	NULL	posttreatment nausea	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , previous research did not test whether motion sickness increases anticipatory nausea only by increasing the base rate of posttreatment nausea and vomiting ( which has traditionally served as the unconditioned stimulus in the conditioning model for anticipatory nausea ) or , alternatively , whether motion sickness might facilitate the association of external stimuli to posttreatment nausea and vomiting .
	manualset3
88557	12	398851	13	NULL	NULL	0	NULL	vomiting	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , previous research did not test whether motion sickness increases anticipatory nausea only by increasing the base rate of posttreatment nausea and vomiting ( which has traditionally served as the unconditioned stimulus in the conditioning model for anticipatory nausea ) or , alternatively , whether motion sickness might facilitate the association of external stimuli to posttreatment nausea and vomiting .
	manualset3
88558	1	398852	13	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , previous studies of Ca ( i ) ( 2 + ) handling have been limited to recordings from the heart surface during short-duration ventricular fibrillation .
	manualset3
88559	2	398852	13	NULL	NULL	0	NULL	Ca ( i ) ( 2 + ) 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	However , previous studies of Ca ( i ) ( 2 + ) handling have been limited to recordings from the heart surface during short-duration ventricular fibrillation .
	manualset3
88560	3	398852	13	NULL	NULL	0	NULL	 recordings 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , previous studies of Ca ( i ) ( 2 + ) handling have been limited to recordings from the heart surface during short-duration ventricular fibrillation .
	manualset3
88561	4	398852	13	NULL	NULL	0	NULL	heart surface 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , previous studies of Ca ( i ) ( 2 + ) handling have been limited to recordings from the heart surface during short-duration ventricular fibrillation .
	manualset3
88562	5	398852	13	NULL	NULL	0	NULL	short-duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	However , previous studies of Ca ( i ) ( 2 + ) handling have been limited to recordings from the heart surface during short-duration ventricular fibrillation .
	manualset3
88563	6	398852	13	NULL	NULL	0	NULL	ventricular fibrillation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , previous studies of Ca ( i ) ( 2 + ) handling have been limited to recordings from the heart surface during short-duration ventricular fibrillation .
	manualset3
88564	1	398853	13	NULL	NULL	0	NULL	period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	However , prolonging the period of breath holding prior to exhalation reduced DLCO ( exhaled ) values at all lung volumes when non-uniform diffusion was simulated , but did not affect DLCO ( exhaled ) when only nonuniform ventilation was simulated .
	manualset3
88565	2	398853	13	NULL	NULL	0	NULL	 breath holding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , prolonging the period of breath holding prior to exhalation reduced DLCO ( exhaled ) values at all lung volumes when non-uniform diffusion was simulated , but did not affect DLCO ( exhaled ) when only nonuniform ventilation was simulated .
	manualset3
88566	3	398853	13	NULL	NULL	0	NULL	exhalation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , prolonging the period of breath holding prior to exhalation reduced DLCO ( exhaled ) values at all lung volumes when non-uniform diffusion was simulated , but did not affect DLCO ( exhaled ) when only nonuniform ventilation was simulated .
	manualset3
88567	4	398853	13	NULL	NULL	0	NULL	DLCO ( exhaled ) values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , prolonging the period of breath holding prior to exhalation reduced DLCO ( exhaled ) values at all lung volumes when non-uniform diffusion was simulated , but did not affect DLCO ( exhaled ) when only nonuniform ventilation was simulated .
	manualset3
88568	5	398853	13	NULL	NULL	0	NULL	lung volumes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , prolonging the period of breath holding prior to exhalation reduced DLCO ( exhaled ) values at all lung volumes when non-uniform diffusion was simulated , but did not affect DLCO ( exhaled ) when only nonuniform ventilation was simulated .
	manualset3
88569	6	398853	13	NULL	NULL	0	NULL	diffusion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , prolonging the period of breath holding prior to exhalation reduced DLCO ( exhaled ) values at all lung volumes when non-uniform diffusion was simulated , but did not affect DLCO ( exhaled ) when only nonuniform ventilation was simulated .
	manualset3
88570	7	398853	13	NULL	NULL	0	NULL	DLCO ( exhaled ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , prolonging the period of breath holding prior to exhalation reduced DLCO ( exhaled ) values at all lung volumes when non-uniform diffusion was simulated , but did not affect DLCO ( exhaled ) when only nonuniform ventilation was simulated .
	manualset3
88571	8	398853	13	NULL	NULL	0	NULL	ventilation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , prolonging the period of breath holding prior to exhalation reduced DLCO ( exhaled ) values at all lung volumes when non-uniform diffusion was simulated , but did not affect DLCO ( exhaled ) when only nonuniform ventilation was simulated .
	manualset3
88572	1	398854	13	NULL	NULL	0	NULL	promoter assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , promoter assays suggest multiple elements present in the p14ARF promoter and argue against the idea that the ARF promoter has a unique ability to distinguish between aberrant and physiological levels of E2F1 .
	manualset3
88573	2	398854	13	NULL	NULL	0	NULL	elements 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	However , promoter assays suggest multiple elements present in the p14ARF promoter and argue against the idea that the ARF promoter has a unique ability to distinguish between aberrant and physiological levels of E2F1 .
	manualset3
88574	3	398854	13	NULL	NULL	0	NULL	p14ARF promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	However , promoter assays suggest multiple elements present in the p14ARF promoter and argue against the idea that the ARF promoter has a unique ability to distinguish between aberrant and physiological levels of E2F1 .
	manualset3
88575	4	398854	13	NULL	NULL	0	NULL	idea	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , promoter assays suggest multiple elements present in the p14ARF promoter and argue against the idea that the ARF promoter has a unique ability to distinguish between aberrant and physiological levels of E2F1 .
	manualset3
88576	5	398854	13	NULL	NULL	0	NULL	ARF promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	However , promoter assays suggest multiple elements present in the p14ARF promoter and argue against the idea that the ARF promoter has a unique ability to distinguish between aberrant and physiological levels of E2F1 .
	manualset3
88577	6	398854	13	NULL	NULL	0	NULL	E2F1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , promoter assays suggest multiple elements present in the p14ARF promoter and argue against the idea that the ARF promoter has a unique ability to distinguish between aberrant and physiological levels of E2F1 .
	manualset3
88578	1	398855	13	NULL	NULL	0	NULL	protein localization studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , protein localization studies show that the R. sphaeroides chemotaxis proteins are organized into two distinct sensory clusters -- one containing transmembrane receptors located at the cell poles and the other containing soluble chemoreceptors located in the cytoplasm .
	manualset3
88579	2	398855	13	NULL	NULL	NULL	NULL	R. sphaeroides chemotaxis proteins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , protein localization studies show that the R. sphaeroides chemotaxis proteins are organized into two distinct sensory clusters -- one containing transmembrane receptors located at the cell poles and the other containing soluble chemoreceptors located in the cytoplasm .
	manualset3
88580	3	398855	13	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , protein localization studies show that the R. sphaeroides chemotaxis proteins are organized into two distinct sensory clusters -- one containing transmembrane receptors located at the cell poles and the other containing soluble chemoreceptors located in the cytoplasm .
	manualset3
88581	4	398855	13	NULL	NULL	0	NULL	sensory clusters 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , protein localization studies show that the R. sphaeroides chemotaxis proteins are organized into two distinct sensory clusters -- one containing transmembrane receptors located at the cell poles and the other containing soluble chemoreceptors located in the cytoplasm .
	manualset3
88582	5	398855	13	NULL	NULL	0	NULL	transmembrane receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , protein localization studies show that the R. sphaeroides chemotaxis proteins are organized into two distinct sensory clusters -- one containing transmembrane receptors located at the cell poles and the other containing soluble chemoreceptors located in the cytoplasm .
	manualset3
88583	6	398855	13	NULL	NULL	0	NULL	 cell poles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	However , protein localization studies show that the R. sphaeroides chemotaxis proteins are organized into two distinct sensory clusters -- one containing transmembrane receptors located at the cell poles and the other containing soluble chemoreceptors located in the cytoplasm .
	manualset3
88584	7	398855	13	NULL	NULL	0	NULL	soluble chemoreceptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , protein localization studies show that the R. sphaeroides chemotaxis proteins are organized into two distinct sensory clusters -- one containing transmembrane receptors located at the cell poles and the other containing soluble chemoreceptors located in the cytoplasm .
	manualset3
88585	8	398855	13	NULL	NULL	0	NULL	cytoplasm	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	However , protein localization studies show that the R. sphaeroides chemotaxis proteins are organized into two distinct sensory clusters -- one containing transmembrane receptors located at the cell poles and the other containing soluble chemoreceptors located in the cytoplasm .
	manualset3
88586	1	398856	13	NULL	NULL	0	NULL	pseudophakia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , pseudophakia changes the physiology of the eye and immediate changes include release of inflammatory cytokines .
	manualset3
88587	2	398856	13	NULL	NULL	0	NULL	physiology 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , pseudophakia changes the physiology of the eye and immediate changes include release of inflammatory cytokines .
	manualset3
88588	3	398856	13	NULL	NULL	0	NULL	 eye 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , pseudophakia changes the physiology of the eye and immediate changes include release of inflammatory cytokines .
	manualset3
88589	4	398856	13	NULL	NULL	0	NULL	inflammatory cytokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , pseudophakia changes the physiology of the eye and immediate changes include release of inflammatory cytokines .
	manualset3
88590	1	398857	13	NULL	NULL	0	NULL	punctal and canalicular agenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , punctal and canalicular agenesis is not among these reported abnormalities .
	manualset3
88591	2	398857	13	NULL	NULL	0	NULL	abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , punctal and canalicular agenesis is not among these reported abnormalities .
	manualset3
88592	1	398858	13	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , recent evidence indicates that , instead , sarcolemmal LCFA transport mediated by CD36 in concert with FABPpm provides a major site of flux control .
	manualset3
88593	2	398858	13	NULL	NULL	0	NULL	sarcolemmal LCFA transport	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , recent evidence indicates that , instead , sarcolemmal LCFA transport mediated by CD36 in concert with FABPpm provides a major site of flux control .
	manualset3
88594	3	398858	13	NULL	NULL	0	NULL	CD36	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , recent evidence indicates that , instead , sarcolemmal LCFA transport mediated by CD36 in concert with FABPpm provides a major site of flux control .
	manualset3
88595	4	398858	13	NULL	NULL	0	NULL	FABPpm	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , recent evidence indicates that , instead , sarcolemmal LCFA transport mediated by CD36 in concert with FABPpm provides a major site of flux control .
	manualset3
88596	5	398858	13	NULL	NULL	0	NULL	site	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , recent evidence indicates that , instead , sarcolemmal LCFA transport mediated by CD36 in concert with FABPpm provides a major site of flux control .
	manualset3
88597	6	398858	13	NULL	NULL	0	NULL	 flux 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , recent evidence indicates that , instead , sarcolemmal LCFA transport mediated by CD36 in concert with FABPpm provides a major site of flux control .
	manualset3
88598	1	398859	13	NULL	NULL	0	NULL	 metal ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effect of metal ions on the phosphate-containing moiety of thrombokinase ) .
	manualset3
88599	2	398859	13	NULL	NULL	0	NULL	phosphate-containing moiety 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effect of metal ions on the phosphate-containing moiety of thrombokinase ) .
	manualset3
88600	3	398859	13	NULL	NULL	0	NULL	 thrombokinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effect of metal ions on the phosphate-containing moiety of thrombokinase ) .
	manualset3
88601	1	398860	13	NULL	NULL	0	NULL	evidence 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , recent evidence suggests a nonredundant unique role for IL-15 in the establishment and perhaps maintenance of peripheral natural killer ( NK ) cell populations in vivo .
	manualset3
88602	2	398860	13	NULL	NULL	0	NULL	IL-15 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , recent evidence suggests a nonredundant unique role for IL-15 in the establishment and perhaps maintenance of peripheral natural killer ( NK ) cell populations in vivo .
	manualset3
88603	3	398860	13	NULL	NULL	0	NULL	establishment 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , recent evidence suggests a nonredundant unique role for IL-15 in the establishment and perhaps maintenance of peripheral natural killer ( NK ) cell populations in vivo .
	manualset3
88604	4	398860	13	NULL	NULL	0	NULL	maintenance 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , recent evidence suggests a nonredundant unique role for IL-15 in the establishment and perhaps maintenance of peripheral natural killer ( NK ) cell populations in vivo .
	manualset3
88605	5	398860	13	NULL	NULL	0	NULL	peripheral natural killer ( NK ) cell populations 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , recent evidence suggests a nonredundant unique role for IL-15 in the establishment and perhaps maintenance of peripheral natural killer ( NK ) cell populations in vivo .
	manualset3
88606	1	398861	13	NULL	NULL	0	NULL	 studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , recent studies suggest that DDAH may regulate eNOS activity and endothelial function through both ADMA-dependent and - independent mechanisms .
	manualset3
88607	2	398861	13	NULL	NULL	0	NULL	DDAH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , recent studies suggest that DDAH may regulate eNOS activity and endothelial function through both ADMA-dependent and - independent mechanisms .
	manualset3
88608	3	398861	13	NULL	NULL	NULL	NULL	eNOS activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , recent studies suggest that DDAH may regulate eNOS activity and endothelial function through both ADMA-dependent and - independent mechanisms .
	manualset3
88609	4	398861	13	NULL	NULL	0	NULL	endothelial function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , recent studies suggest that DDAH may regulate eNOS activity and endothelial function through both ADMA-dependent and - independent mechanisms .
	manualset3
88610	5	398861	13	NULL	NULL	0	NULL	ADMA-dependent mechanisms 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , recent studies suggest that DDAH may regulate eNOS activity and endothelial function through both ADMA-dependent and - independent mechanisms .
	manualset3
88611	6	398861	13	NULL	NULL	NULL	NULL	ADMA-independent mechanisms	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , recent studies suggest that DDAH may regulate eNOS activity and endothelial function through both ADMA-dependent and - independent mechanisms .
	manualset3
88612	1	398862	13	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , results from in-gel and Western blot analysis suggested that expression of recombinant GsiA in Rosetta ( DE3 ) provides an efficient source in soluble form .
	manualset3
88613	2	398862	13	NULL	NULL	0	NULL	in-gel analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , results from in-gel and Western blot analysis suggested that expression of recombinant GsiA in Rosetta ( DE3 ) provides an efficient source in soluble form .
	manualset3
88614	3	398862	13	NULL	NULL	0	NULL	Western blot analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , results from in-gel and Western blot analysis suggested that expression of recombinant GsiA in Rosetta ( DE3 ) provides an efficient source in soluble form .
	manualset3
88615	4	398862	13	NULL	NULL	0	NULL	 expression of recombinant GsiA	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , results from in-gel and Western blot analysis suggested that expression of recombinant GsiA in Rosetta ( DE3 ) provides an efficient source in soluble form .
	manualset3
88616	5	398862	13	NULL	NULL	0	NULL	Rosetta ( DE3 ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , results from in-gel and Western blot analysis suggested that expression of recombinant GsiA in Rosetta ( DE3 ) provides an efficient source in soluble form .
	manualset3
88617	6	398862	13	NULL	NULL	0	NULL	source	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , results from in-gel and Western blot analysis suggested that expression of recombinant GsiA in Rosetta ( DE3 ) provides an efficient source in soluble form .
	manualset3
88618	1	398863	13	NULL	NULL	0	NULL	 banding procedures	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , routine banding procedures , by themselves , provide only limited information about the identity of marker chromosomes .
	manualset3
88619	2	398863	13	NULL	NULL	0	NULL	information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , routine banding procedures , by themselves , provide only limited information about the identity of marker chromosomes .
	manualset3
88620	3	398863	13	NULL	NULL	0	NULL	 marker chromosomes	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	However , routine banding procedures , by themselves , provide only limited information about the identity of marker chromosomes .
	manualset3
88621	1	398864	13	NULL	NULL	0	NULL	schizophrenia diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , schizophrenia diagnosis was a strong predictor ( p & lt ; 0.0005 ) of the abundance of a truncated 50 kDa GR protein isoform , putative GR-D1 , which was increased in schizophrenia cases ( 80.4 % ) relative to controls .
	manualset3
88622	2	398864	13	NULL	NULL	0	NULL	predictor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , schizophrenia diagnosis was a strong predictor ( p & lt ; 0.0005 ) of the abundance of a truncated 50 kDa GR protein isoform , putative GR-D1 , which was increased in schizophrenia cases ( 80.4 % ) relative to controls .
	manualset3
88623	3	398864	13	NULL	NULL	0	NULL	 p & lt ; 0.0005 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , schizophrenia diagnosis was a strong predictor ( p & lt ; 0.0005 ) of the abundance of a truncated 50 kDa GR protein isoform , putative GR-D1 , which was increased in schizophrenia cases ( 80.4 % ) relative to controls .
	manualset3
88624	4	398864	13	NULL	NULL	0	NULL	truncated 50 kDa GR protein isoform	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , schizophrenia diagnosis was a strong predictor ( p & lt ; 0.0005 ) of the abundance of a truncated 50 kDa GR protein isoform , putative GR-D1 , which was increased in schizophrenia cases ( 80.4 % ) relative to controls .
	manualset3
88625	5	398864	13	NULL	NULL	0	NULL	putative GR-D1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , schizophrenia diagnosis was a strong predictor ( p & lt ; 0.0005 ) of the abundance of a truncated 50 kDa GR protein isoform , putative GR-D1 , which was increased in schizophrenia cases ( 80.4 % ) relative to controls .
	manualset3
88626	6	398864	13	NULL	NULL	0	NULL	schizophrenia cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , schizophrenia diagnosis was a strong predictor ( p & lt ; 0.0005 ) of the abundance of a truncated 50 kDa GR protein isoform , putative GR-D1 , which was increased in schizophrenia cases ( 80.4 % ) relative to controls .
	manualset3
88627	7	398864	13	NULL	NULL	0	NULL	80.4 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , schizophrenia diagnosis was a strong predictor ( p & lt ; 0.0005 ) of the abundance of a truncated 50 kDa GR protein isoform , putative GR-D1 , which was increased in schizophrenia cases ( 80.4 % ) relative to controls .
	manualset3
88628	8	398864	13	NULL	NULL	0	NULL	 controls 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , schizophrenia diagnosis was a strong predictor ( p & lt ; 0.0005 ) of the abundance of a truncated 50 kDa GR protein isoform , putative GR-D1 , which was increased in schizophrenia cases ( 80.4 % ) relative to controls .
	manualset3
88629	1	398865	13	NULL	NULL	NULL	NULL	scopolamine 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , scopolamine dose-dependently facilitated the striatal ECF dopamine induced by the DAT inhibitor GBR12909 at a dose of 0.5 mg/kg .
	manualset3
88630	2	398865	13	NULL	NULL	0	NULL	striatal ECF dopamine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , scopolamine dose-dependently facilitated the striatal ECF dopamine induced by the DAT inhibitor GBR12909 at a dose of 0.5 mg/kg .
	manualset3
88631	3	398865	13	NULL	NULL	0	NULL	DAT inhibitor GBR12909	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , scopolamine dose-dependently facilitated the striatal ECF dopamine induced by the DAT inhibitor GBR12909 at a dose of 0.5 mg/kg .
	manualset3
88632	4	398865	13	NULL	NULL	0	NULL	dose of 0.5 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , scopolamine dose-dependently facilitated the striatal ECF dopamine induced by the DAT inhibitor GBR12909 at a dose of 0.5 mg/kg .
	manualset3
88784	1	398866	13	NULL	NULL	0	NULL	weight control program	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effects of a weight control program with competence ) .
	manualset3
88785	2	398866	13	NULL	NULL	0	NULL	competence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effects of a weight control program with competence ) .
	manualset3
88788	1	398867	13	NULL	NULL	0	NULL	screening	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , screening for antituberculosis compounds by using GFP driven by the heat shock promoter , hsp60 , has been of limited utility due to the low signal-to-noise ratio .
	manualset3
88795	2	398867	13	NULL	NULL	0	NULL	antituberculosis compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , screening for antituberculosis compounds by using GFP driven by the heat shock promoter , hsp60 , has been of limited utility due to the low signal-to-noise ratio .
	manualset3
88796	3	398867	13	NULL	NULL	0	NULL	GFP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , screening for antituberculosis compounds by using GFP driven by the heat shock promoter , hsp60 , has been of limited utility due to the low signal-to-noise ratio .
	manualset3
88800	4	398867	13	NULL	NULL	NULL	NULL	heat shock promoter , hsp60	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , screening for antituberculosis compounds by using GFP driven by the heat shock promoter , hsp60 , has been of limited utility due to the low signal-to-noise ratio .
	manualset3
88805	5	398867	13	NULL	NULL	0	NULL	signal-to-noise ratio	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , screening for antituberculosis compounds by using GFP driven by the heat shock promoter , hsp60 , has been of limited utility due to the low signal-to-noise ratio .
	manualset3
88837	1	398868	13	NULL	NULL	NULL	NULL	sensory tuning properties	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , sensory tuning properties in these areas , especially during wakefulness , and their relation to perception , are poorly understood .
	manualset3
88838	2	398868	13	NULL	NULL	0	NULL	areas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , sensory tuning properties in these areas , especially during wakefulness , and their relation to perception , are poorly understood .
	manualset3
88846	3	398868	13	NULL	NULL	0	NULL	wakefulness	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , sensory tuning properties in these areas , especially during wakefulness , and their relation to perception , are poorly understood .
	manualset3
88847	4	398868	13	NULL	NULL	NULL	NULL	perception 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , sensory tuning properties in these areas , especially during wakefulness , and their relation to perception , are poorly understood .
	manualset3
88849	1	398869	13	NULL	NULL	0	NULL	dysarthria 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , severe dysarthria and myoclonic jerks in a patient with hemiparesis should be considered as warning signs to indicate the herald hemiparesis with subsequent severe brainstem infarction .
	manualset3
88850	2	398869	13	NULL	NULL	0	NULL	myoclonic jerks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , severe dysarthria and myoclonic jerks in a patient with hemiparesis should be considered as warning signs to indicate the herald hemiparesis with subsequent severe brainstem infarction .
	manualset3
88852	3	398869	13	NULL	NULL	0	NULL	patient	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , severe dysarthria and myoclonic jerks in a patient with hemiparesis should be considered as warning signs to indicate the herald hemiparesis with subsequent severe brainstem infarction .
	manualset3
88856	4	398869	13	NULL	NULL	0	NULL	hemiparesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , severe dysarthria and myoclonic jerks in a patient with hemiparesis should be considered as warning signs to indicate the herald hemiparesis with subsequent severe brainstem infarction .
	manualset3
88861	5	398869	13	NULL	NULL	0	NULL	warning signs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , severe dysarthria and myoclonic jerks in a patient with hemiparesis should be considered as warning signs to indicate the herald hemiparesis with subsequent severe brainstem infarction .
	manualset3
88862	6	398869	13	NULL	NULL	0	NULL	herald hemiparesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , severe dysarthria and myoclonic jerks in a patient with hemiparesis should be considered as warning signs to indicate the herald hemiparesis with subsequent severe brainstem infarction .
	manualset3
88863	7	398869	13	NULL	NULL	0	NULL	severe brainstem infarction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , severe dysarthria and myoclonic jerks in a patient with hemiparesis should be considered as warning signs to indicate the herald hemiparesis with subsequent severe brainstem infarction .
	manualset3
88864	1	398870	13	NULL	NULL	0	NULL	cross-protection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , significant cross-protection was observed when serotype II and III strains were analyzed in the model .
	manualset3
88865	2	398870	13	NULL	NULL	0	NULL	serotype II strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , significant cross-protection was observed when serotype II and III strains were analyzed in the model .
	manualset3
88866	3	398870	13	NULL	NULL	0	NULL	serotype III strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , significant cross-protection was observed when serotype II and III strains were analyzed in the model .
	manualset3
88867	4	398870	13	NULL	NULL	NULL	NULL	model	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , significant cross-protection was observed when serotype II and III strains were analyzed in the model .
	manualset3
88868	1	398871	13	NULL	NULL	0	NULL	RT-PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , since RT-PCR generally lacks the specificity of sequencing or serology , the most practical application of RT-PCR methods for subtype identification is either to target a few of the most important subtypes such as H5 and H7 or to use it in situations where a specific strain is being targeted , such as during an outbreak or with experimental samples .
	manualset3
88872	2	398871	13	NULL	NULL	0	NULL	sequencing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , since RT-PCR generally lacks the specificity of sequencing or serology , the most practical application of RT-PCR methods for subtype identification is either to target a few of the most important subtypes such as H5 and H7 or to use it in situations where a specific strain is being targeted , such as during an outbreak or with experimental samples .
	manualset3
88873	3	398871	13	NULL	NULL	NULL	NULL	serology	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , since RT-PCR generally lacks the specificity of sequencing or serology , the most practical application of RT-PCR methods for subtype identification is either to target a few of the most important subtypes such as H5 and H7 or to use it in situations where a specific strain is being targeted , such as during an outbreak or with experimental samples .
	manualset3
88875	4	398871	13	NULL	NULL	0	NULL	RT-PCR methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , since RT-PCR generally lacks the specificity of sequencing or serology , the most practical application of RT-PCR methods for subtype identification is either to target a few of the most important subtypes such as H5 and H7 or to use it in situations where a specific strain is being targeted , such as during an outbreak or with experimental samples .
	manualset3
88876	5	398871	13	NULL	NULL	0	NULL	subtype identification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , since RT-PCR generally lacks the specificity of sequencing or serology , the most practical application of RT-PCR methods for subtype identification is either to target a few of the most important subtypes such as H5 and H7 or to use it in situations where a specific strain is being targeted , such as during an outbreak or with experimental samples .
	manualset3
88881	6	398871	13	NULL	NULL	0	NULL	H5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , since RT-PCR generally lacks the specificity of sequencing or serology , the most practical application of RT-PCR methods for subtype identification is either to target a few of the most important subtypes such as H5 and H7 or to use it in situations where a specific strain is being targeted , such as during an outbreak or with experimental samples .
	manualset3
88882	7	398871	13	NULL	NULL	0	NULL	H7	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , since RT-PCR generally lacks the specificity of sequencing or serology , the most practical application of RT-PCR methods for subtype identification is either to target a few of the most important subtypes such as H5 and H7 or to use it in situations where a specific strain is being targeted , such as during an outbreak or with experimental samples .
	manualset3
88883	8	398871	13	NULL	NULL	0	NULL	strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , since RT-PCR generally lacks the specificity of sequencing or serology , the most practical application of RT-PCR methods for subtype identification is either to target a few of the most important subtypes such as H5 and H7 or to use it in situations where a specific strain is being targeted , such as during an outbreak or with experimental samples .
	manualset3
88884	9	398871	13	NULL	NULL	0	NULL	outbreak 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , since RT-PCR generally lacks the specificity of sequencing or serology , the most practical application of RT-PCR methods for subtype identification is either to target a few of the most important subtypes such as H5 and H7 or to use it in situations where a specific strain is being targeted , such as during an outbreak or with experimental samples .
	manualset3
88885	10	398871	13	NULL	NULL	0	NULL	experimental samples 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , since RT-PCR generally lacks the specificity of sequencing or serology , the most practical application of RT-PCR methods for subtype identification is either to target a few of the most important subtypes such as H5 and H7 or to use it in situations where a specific strain is being targeted , such as during an outbreak or with experimental samples .
	manualset3
88900	1	398872	13	NULL	NULL	NULL	NULL	 immobilization	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , single immobilization significantly decreased beta ( 2 ) - AR mRNA levels both in left atria and ventricles compared to acute cold stress .
	manualset3
88901	2	398872	13	NULL	NULL	0	NULL	beta ( 2 ) - AR mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	However , single immobilization significantly decreased beta ( 2 ) - AR mRNA levels both in left atria and ventricles compared to acute cold stress .
	manualset3
88902	3	398872	13	NULL	NULL	0	NULL	left atria	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , single immobilization significantly decreased beta ( 2 ) - AR mRNA levels both in left atria and ventricles compared to acute cold stress .
	manualset3
88903	4	398872	13	NULL	NULL	0	NULL	ventricles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , single immobilization significantly decreased beta ( 2 ) - AR mRNA levels both in left atria and ventricles compared to acute cold stress .
	manualset3
88904	5	398872	13	NULL	NULL	0	NULL	cold stress	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , single immobilization significantly decreased beta ( 2 ) - AR mRNA levels both in left atria and ventricles compared to acute cold stress .
	manualset3
88905	1	398873	13	NULL	NULL	0	NULL	 sodium channels	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , sodium channels were detected only in axon patches .
	manualset3
88906	2	398873	13	NULL	NULL	0	NULL	axon patches	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , sodium channels were detected only in axon patches .
	manualset3
88907	1	398874	13	NULL	NULL	0	NULL	activities 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , some activities were located in high molecular weight complexes , and methods that disrupted these complexes ( such as treatment with sodium dodecyl sulfate at elevated temperature ) destroyed enzyme activity .
	manualset3
88908	2	398874	13	NULL	NULL	0	NULL	 high molecular weight complexes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , some activities were located in high molecular weight complexes , and methods that disrupted these complexes ( such as treatment with sodium dodecyl sulfate at elevated temperature ) destroyed enzyme activity .
	manualset3
88909	3	398874	13	NULL	NULL	NULL	NULL	methods	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , some activities were located in high molecular weight complexes , and methods that disrupted these complexes ( such as treatment with sodium dodecyl sulfate at elevated temperature ) destroyed enzyme activity .
	manualset3
88910	4	398874	13	NULL	NULL	0	NULL	complexes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , some activities were located in high molecular weight complexes , and methods that disrupted these complexes ( such as treatment with sodium dodecyl sulfate at elevated temperature ) destroyed enzyme activity .
	manualset3
88911	5	398874	13	NULL	NULL	0	NULL	treatment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , some activities were located in high molecular weight complexes , and methods that disrupted these complexes ( such as treatment with sodium dodecyl sulfate at elevated temperature ) destroyed enzyme activity .
	manualset3
88912	6	398874	13	NULL	NULL	0	NULL	sodium dodecyl sulfate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , some activities were located in high molecular weight complexes , and methods that disrupted these complexes ( such as treatment with sodium dodecyl sulfate at elevated temperature ) destroyed enzyme activity .
	manualset3
88913	7	398874	13	NULL	NULL	0	NULL	temperature 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , some activities were located in high molecular weight complexes , and methods that disrupted these complexes ( such as treatment with sodium dodecyl sulfate at elevated temperature ) destroyed enzyme activity .
	manualset3
88914	8	398874	13	NULL	NULL	0	NULL	enzyme activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , some activities were located in high molecular weight complexes , and methods that disrupted these complexes ( such as treatment with sodium dodecyl sulfate at elevated temperature ) destroyed enzyme activity .
	manualset3
88915	1	398875	13	NULL	NULL	NULL	NULL	 effects	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The effects of iodized sodium tetrachloride on certain fungi ) .
	manualset3
88916	2	398875	13	NULL	NULL	0	NULL	iodized sodium tetrachloride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effects of iodized sodium tetrachloride on certain fungi ) .
	manualset3
88917	3	398875	13	NULL	NULL	0	NULL	fungi 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effects of iodized sodium tetrachloride on certain fungi ) .
	manualset3
88918	1	398876	13	NULL	NULL	0	NULL	targets	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , specific targets for calmodulin action have not been thoroughly addressed .
	manualset3
88919	2	398876	13	NULL	NULL	0	NULL	calmodulin action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , specific targets for calmodulin action have not been thoroughly addressed .
	manualset3
88920	1	398877	13	NULL	NULL	0	NULL	 neurotransmitter release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , spontaneous neurotransmitter release was stable ( both in frequency and amplitude ) throughout the period of antibody exposure .
	manualset3
88921	2	398877	13	NULL	NULL	0	NULL	frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , spontaneous neurotransmitter release was stable ( both in frequency and amplitude ) throughout the period of antibody exposure .
	manualset3
88922	3	398877	13	NULL	NULL	0	NULL	 amplitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , spontaneous neurotransmitter release was stable ( both in frequency and amplitude ) throughout the period of antibody exposure .
	manualset3
88923	4	398877	13	NULL	NULL	0	NULL	period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	However , spontaneous neurotransmitter release was stable ( both in frequency and amplitude ) throughout the period of antibody exposure .
	manualset3
88924	5	398877	13	NULL	NULL	NULL	NULL	antibody	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , spontaneous neurotransmitter release was stable ( both in frequency and amplitude ) throughout the period of antibody exposure .
	manualset3
88926	6	398877	13	NULL	NULL	0	NULL	exposure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , spontaneous neurotransmitter release was stable ( both in frequency and amplitude ) throughout the period of antibody exposure .
	manualset3
88927	1	398878	13	NULL	NULL	0	NULL	 statistical analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , statistical analyses substantiated the observation that the bases of the sinuses and raphes were the valvular regions particularly prone to the development of cartilage .
	manualset3
88928	2	398878	13	NULL	NULL	0	NULL	observation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , statistical analyses substantiated the observation that the bases of the sinuses and raphes were the valvular regions particularly prone to the development of cartilage .
	manualset3
88929	3	398878	13	NULL	NULL	NULL	NULL	bases of the sinuses	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , statistical analyses substantiated the observation that the bases of the sinuses and raphes were the valvular regions particularly prone to the development of cartilage .
	manualset3
88930	4	398878	13	NULL	NULL	0	NULL	raphes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , statistical analyses substantiated the observation that the bases of the sinuses and raphes were the valvular regions particularly prone to the development of cartilage .
	manualset3
88931	5	398878	13	NULL	NULL	0	NULL	valvular regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , statistical analyses substantiated the observation that the bases of the sinuses and raphes were the valvular regions particularly prone to the development of cartilage .
	manualset3
88932	6	398878	13	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , statistical analyses substantiated the observation that the bases of the sinuses and raphes were the valvular regions particularly prone to the development of cartilage .
	manualset3
88933	7	398878	13	NULL	NULL	0	NULL	cartilage	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	However , statistical analyses substantiated the observation that the bases of the sinuses and raphes were the valvular regions particularly prone to the development of cartilage .
	manualset3
88934	1	398879	13	NULL	NULL	0	NULL	structurally and mechanistically dissimilar inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , structurally and mechanistically dissimilar inhibitors of protein methylation and coexpression of protein arginine methyltransferase 1 did not influence Nox activity .
	manualset3
88941	2	398879	13	NULL	NULL	0	NULL	protein methylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , structurally and mechanistically dissimilar inhibitors of protein methylation and coexpression of protein arginine methyltransferase 1 did not influence Nox activity .
	manualset3
88942	3	398879	13	NULL	NULL	0	NULL	coexpression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , structurally and mechanistically dissimilar inhibitors of protein methylation and coexpression of protein arginine methyltransferase 1 did not influence Nox activity .
	manualset3
88943	4	398879	13	NULL	NULL	0	NULL	 protein arginine methyltransferase 1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , structurally and mechanistically dissimilar inhibitors of protein methylation and coexpression of protein arginine methyltransferase 1 did not influence Nox activity .
	manualset3
88944	5	398879	13	NULL	NULL	0	NULL	Nox activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , structurally and mechanistically dissimilar inhibitors of protein methylation and coexpression of protein arginine methyltransferase 1 did not influence Nox activity .
	manualset3
90008	6	398879	13	NULL	NULL	0	NULL	influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , structurally and mechanistically dissimilar inhibitors of protein methylation and coexpression of protein arginine methyltransferase 1 did not influence Nox activity .
	manualset3
88945	1	398880	13	NULL	NULL	0	NULL	interconnections	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , such interconnections have remained elusive due to the difficulty in separating the intra - and extraribosomal roles of ribosome biogenesis factors .
	manualset3
88946	2	398880	13	NULL	NULL	0	NULL	intraribosomal roles	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , such interconnections have remained elusive due to the difficulty in separating the intra - and extraribosomal roles of ribosome biogenesis factors .
	manualset3
88947	3	398880	13	NULL	NULL	0	NULL	extraribosomal roles	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , such interconnections have remained elusive due to the difficulty in separating the intra - and extraribosomal roles of ribosome biogenesis factors .
	manualset3
88948	4	398880	13	NULL	NULL	0	NULL	ribosome biogenesis factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , such interconnections have remained elusive due to the difficulty in separating the intra - and extraribosomal roles of ribosome biogenesis factors .
	manualset3
88949	1	398881	13	NULL	NULL	NULL	NULL	support 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , such support was predicated on the specialty 's highlighting particular legitimating discourses and practices at the expense of others , and in framing this in terms of specific policy concerns around an ageing population .
	manualset3
88950	2	398881	13	NULL	NULL	0	NULL	discourses	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , such support was predicated on the specialty 's highlighting particular legitimating discourses and practices at the expense of others , and in framing this in terms of specific policy concerns around an ageing population .
	manualset3
88951	3	398881	13	NULL	NULL	0	NULL	practices	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , such support was predicated on the specialty 's highlighting particular legitimating discourses and practices at the expense of others , and in framing this in terms of specific policy concerns around an ageing population .
	manualset3
88952	4	398881	13	NULL	NULL	0	NULL	policy	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , such support was predicated on the specialty 's highlighting particular legitimating discourses and practices at the expense of others , and in framing this in terms of specific policy concerns around an ageing population .
	manualset3
88953	5	398881	13	NULL	NULL	0	NULL	ageing population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , such support was predicated on the specialty 's highlighting particular legitimating discourses and practices at the expense of others , and in framing this in terms of specific policy concerns around an ageing population .
	manualset3
88954	1	398882	13	NULL	NULL	0	NULL	sulphated insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , sulphated insulin bound to liver membranes with an affinity more closely resembling that for adipocytes rather than hepatocytes .
	manualset3
88955	2	398882	13	NULL	NULL	0	NULL	liver membranes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , sulphated insulin bound to liver membranes with an affinity more closely resembling that for adipocytes rather than hepatocytes .
	manualset3
88956	3	398882	13	NULL	NULL	0	NULL	affinity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , sulphated insulin bound to liver membranes with an affinity more closely resembling that for adipocytes rather than hepatocytes .
	manualset3
88957	4	398882	13	NULL	NULL	0	NULL	adipocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , sulphated insulin bound to liver membranes with an affinity more closely resembling that for adipocytes rather than hepatocytes .
	manualset3
88958	5	398882	13	NULL	NULL	0	NULL	hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , sulphated insulin bound to liver membranes with an affinity more closely resembling that for adipocytes rather than hepatocytes .
	manualset3
88959	1	398883	13	NULL	NULL	0	NULL	synaptic circuit mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , synaptic circuit mechanisms underlying the OS sharpening remain unclear .
	manualset3
88960	2	398883	13	NULL	NULL	0	NULL	OS sharpening 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , synaptic circuit mechanisms underlying the OS sharpening remain unclear .
	manualset3
88961	1	398884	13	NULL	NULL	0	NULL	syncollin-deficient mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , syncollin-deficient mice reacted to caerulein hyperstimulation with a more severe pancreatitis .
	manualset3
88962	2	398884	13	NULL	NULL	0	NULL	caerulein	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	However , syncollin-deficient mice reacted to caerulein hyperstimulation with a more severe pancreatitis .
	manualset3
88963	3	398884	13	NULL	NULL	0	NULL	hyperstimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , syncollin-deficient mice reacted to caerulein hyperstimulation with a more severe pancreatitis .
	manualset3
88964	4	398884	13	NULL	NULL	0	NULL	pancreatitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , syncollin-deficient mice reacted to caerulein hyperstimulation with a more severe pancreatitis .
	manualset3
88965	1	398885	13	NULL	NULL	0	NULL	etiology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( The etiology of chronic anti-HBc-positive hepatitis ) .
	manualset3
88966	2	398885	13	NULL	NULL	0	NULL	 chronic anti-HBc-positive hepatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( The etiology of chronic anti-HBc-positive hepatitis ) .
	manualset3
88967	1	398886	13	NULL	NULL	0	NULL	telmisartan	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , telmisartan showed better tolerability than ramipril in ONTARGET , with less cough and angioedema .
	manualset3
88968	2	398886	13	NULL	NULL	0	NULL	tolerability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , telmisartan showed better tolerability than ramipril in ONTARGET , with less cough and angioedema .
	manualset3
88969	3	398886	13	NULL	NULL	0	NULL	ramipril	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , telmisartan showed better tolerability than ramipril in ONTARGET , with less cough and angioedema .
	manualset3
88970	4	398886	13	NULL	NULL	0	NULL	ONTARGET	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , telmisartan showed better tolerability than ramipril in ONTARGET , with less cough and angioedema .
	manualset3
88971	5	398886	13	NULL	NULL	0	NULL	cough 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , telmisartan showed better tolerability than ramipril in ONTARGET , with less cough and angioedema .
	manualset3
88972	6	398886	13	NULL	NULL	0	NULL	angioedema	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , telmisartan showed better tolerability than ramipril in ONTARGET , with less cough and angioedema .
	manualset3
88973	1	398887	13	NULL	NULL	0	NULL	 CGN treatments	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the CGN treatments did not affect the antibody response to BA nor to SRBC differently between L and H line chicks .
	manualset3
88974	2	398887	13	NULL	NULL	NULL	NULL	antibody response	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the CGN treatments did not affect the antibody response to BA nor to SRBC differently between L and H line chicks .
	manualset3
88975	3	398887	13	NULL	NULL	0	NULL	BA	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the CGN treatments did not affect the antibody response to BA nor to SRBC differently between L and H line chicks .
	manualset3
88976	4	398887	13	NULL	NULL	0	NULL	 SRBC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the CGN treatments did not affect the antibody response to BA nor to SRBC differently between L and H line chicks .
	manualset3
88977	5	398887	13	NULL	NULL	0	NULL	L line chicks	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the CGN treatments did not affect the antibody response to BA nor to SRBC differently between L and H line chicks .
	manualset3
88978	6	398887	13	NULL	NULL	0	NULL	H line chicks	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the CGN treatments did not affect the antibody response to BA nor to SRBC differently between L and H line chicks .
	manualset3
89028	1	398888	13	NULL	NULL	0	NULL	ISO/IEC Guide 58	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the ISO/IEC Guide 58 , for the setting up and operation of a laboratory accreditation body , specifies that inspectors should have appropriate technical knowledge of the specific calibrations , tests or types of calibration or tests for which accreditation is sought .
	manualset3
89035	3	398888	13	NULL	NULL	0	NULL	operation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the ISO/IEC Guide 58 , for the setting up and operation of a laboratory accreditation body , specifies that inspectors should have appropriate technical knowledge of the specific calibrations , tests or types of calibration or tests for which accreditation is sought .
	manualset3
89049	4	398888	13	NULL	NULL	0	NULL	laboratory accreditation body	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the ISO/IEC Guide 58 , for the setting up and operation of a laboratory accreditation body , specifies that inspectors should have appropriate technical knowledge of the specific calibrations , tests or types of calibration or tests for which accreditation is sought .
	manualset3
89050	5	398888	13	NULL	NULL	0	NULL	inspectors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the ISO/IEC Guide 58 , for the setting up and operation of a laboratory accreditation body , specifies that inspectors should have appropriate technical knowledge of the specific calibrations , tests or types of calibration or tests for which accreditation is sought .
	manualset3
89052	6	398888	13	NULL	NULL	0	NULL	 technical knowledge 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the ISO/IEC Guide 58 , for the setting up and operation of a laboratory accreditation body , specifies that inspectors should have appropriate technical knowledge of the specific calibrations , tests or types of calibration or tests for which accreditation is sought .
	manualset3
89053	7	398888	13	NULL	NULL	0	NULL	 calibrations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the ISO/IEC Guide 58 , for the setting up and operation of a laboratory accreditation body , specifies that inspectors should have appropriate technical knowledge of the specific calibrations , tests or types of calibration or tests for which accreditation is sought .
	manualset3
89055	8	398888	13	NULL	NULL	0	NULL	tests	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the ISO/IEC Guide 58 , for the setting up and operation of a laboratory accreditation body , specifies that inspectors should have appropriate technical knowledge of the specific calibrations , tests or types of calibration or tests for which accreditation is sought .
	manualset3
89056	9	398888	13	NULL	NULL	0	NULL	calibration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the ISO/IEC Guide 58 , for the setting up and operation of a laboratory accreditation body , specifies that inspectors should have appropriate technical knowledge of the specific calibrations , tests or types of calibration or tests for which accreditation is sought .
	manualset3
89057	10	398888	13	NULL	NULL	0	NULL	tests 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the ISO/IEC Guide 58 , for the setting up and operation of a laboratory accreditation body , specifies that inspectors should have appropriate technical knowledge of the specific calibrations , tests or types of calibration or tests for which accreditation is sought .
	manualset3
89058	11	398888	13	NULL	NULL	0	NULL	accreditation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the ISO/IEC Guide 58 , for the setting up and operation of a laboratory accreditation body , specifies that inspectors should have appropriate technical knowledge of the specific calibrations , tests or types of calibration or tests for which accreditation is sought .
	manualset3
89066	1	398889	13	NULL	NULL	0	NULL	Kcec values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the Kcec values of the enkephalin peptides under all temperature conditions studied were positive with an eluent composed of water-50 mM NH4OAc/AcOH , pH 5.2-acetonitrile ( 5 : 2 : 3 , v/v ) and therefore the chromatographic component dominates the retention process with these small peptides under these conditions .
	manualset3
89067	2	398889	13	NULL	NULL	0	NULL	enkephalin peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the Kcec values of the enkephalin peptides under all temperature conditions studied were positive with an eluent composed of water-50 mM NH4OAc/AcOH , pH 5.2-acetonitrile ( 5 : 2 : 3 , v/v ) and therefore the chromatographic component dominates the retention process with these small peptides under these conditions .
	manualset3
89069	3	398889	13	NULL	NULL	0	NULL	temperature conditions	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the Kcec values of the enkephalin peptides under all temperature conditions studied were positive with an eluent composed of water-50 mM NH4OAc/AcOH , pH 5.2-acetonitrile ( 5 : 2 : 3 , v/v ) and therefore the chromatographic component dominates the retention process with these small peptides under these conditions .
	manualset3
89071	5	398889	13	NULL	NULL	NULL	NULL	water-50 mM NH4OAc/AcOH	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the Kcec values of the enkephalin peptides under all temperature conditions studied were positive with an eluent composed of water-50 mM NH4OAc/AcOH , pH 5.2-acetonitrile ( 5 : 2 : 3 , v/v ) and therefore the chromatographic component dominates the retention process with these small peptides under these conditions .
	manualset3
89074	8	398889	13	NULL	NULL	0	NULL	pH 5.2	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the Kcec values of the enkephalin peptides under all temperature conditions studied were positive with an eluent composed of water-50 mM NH4OAc/AcOH , pH 5.2-acetonitrile ( 5 : 2 : 3 , v/v ) and therefore the chromatographic component dominates the retention process with these small peptides under these conditions .
	manualset3
89078	9	398889	13	NULL	NULL	0	NULL	acetonitrile 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the Kcec values of the enkephalin peptides under all temperature conditions studied were positive with an eluent composed of water-50 mM NH4OAc/AcOH , pH 5.2-acetonitrile ( 5 : 2 : 3 , v/v ) and therefore the chromatographic component dominates the retention process with these small peptides under these conditions .
	manualset3
89079	10	398889	13	NULL	NULL	0	NULL	5 : 2 : 3 , v/v	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the Kcec values of the enkephalin peptides under all temperature conditions studied were positive with an eluent composed of water-50 mM NH4OAc/AcOH , pH 5.2-acetonitrile ( 5 : 2 : 3 , v/v ) and therefore the chromatographic component dominates the retention process with these small peptides under these conditions .
	manualset3
89081	11	398889	13	NULL	NULL	0	NULL	component	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the Kcec values of the enkephalin peptides under all temperature conditions studied were positive with an eluent composed of water-50 mM NH4OAc/AcOH , pH 5.2-acetonitrile ( 5 : 2 : 3 , v/v ) and therefore the chromatographic component dominates the retention process with these small peptides under these conditions .
	manualset3
89082	12	398889	13	NULL	NULL	0	NULL	retention process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the Kcec values of the enkephalin peptides under all temperature conditions studied were positive with an eluent composed of water-50 mM NH4OAc/AcOH , pH 5.2-acetonitrile ( 5 : 2 : 3 , v/v ) and therefore the chromatographic component dominates the retention process with these small peptides under these conditions .
	manualset3
89083	13	398889	13	NULL	NULL	0	NULL	peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the Kcec values of the enkephalin peptides under all temperature conditions studied were positive with an eluent composed of water-50 mM NH4OAc/AcOH , pH 5.2-acetonitrile ( 5 : 2 : 3 , v/v ) and therefore the chromatographic component dominates the retention process with these small peptides under these conditions .
	manualset3
89086	14	398889	13	NULL	NULL	0	NULL	conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the Kcec values of the enkephalin peptides under all temperature conditions studied were positive with an eluent composed of water-50 mM NH4OAc/AcOH , pH 5.2-acetonitrile ( 5 : 2 : 3 , v/v ) and therefore the chromatographic component dominates the retention process with these small peptides under these conditions .
	manualset3
89087	1	398890	13	NULL	NULL	0	NULL	NR3B mRNA expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the NR3B mRNA expression was significantly up-regulated by the factors 9.11 ( P & lt ; 0.001 ) , 10.07 ( P & lt ; 0.001 ) and 4.08 ( P & lt ; 0.05 ) in abstinent , addicted and methadone maintained subjects , respectively relative to control group .
	manualset3
89090	2	398890	13	NULL	NULL	0	NULL	9.11 ( P & lt ; 0.001 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the NR3B mRNA expression was significantly up-regulated by the factors 9.11 ( P & lt ; 0.001 ) , 10.07 ( P & lt ; 0.001 ) and 4.08 ( P & lt ; 0.05 ) in abstinent , addicted and methadone maintained subjects , respectively relative to control group .
	manualset3
89091	3	398890	13	NULL	NULL	0	NULL	 10.07 ( P & lt ; 0.001 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the NR3B mRNA expression was significantly up-regulated by the factors 9.11 ( P & lt ; 0.001 ) , 10.07 ( P & lt ; 0.001 ) and 4.08 ( P & lt ; 0.05 ) in abstinent , addicted and methadone maintained subjects , respectively relative to control group .
	manualset3
89092	4	398890	13	NULL	NULL	0	NULL	4.08 ( P & lt ; 0.05 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the NR3B mRNA expression was significantly up-regulated by the factors 9.11 ( P & lt ; 0.001 ) , 10.07 ( P & lt ; 0.001 ) and 4.08 ( P & lt ; 0.05 ) in abstinent , addicted and methadone maintained subjects , respectively relative to control group .
	manualset3
89093	5	398890	13	NULL	NULL	0	NULL	abstinent subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the NR3B mRNA expression was significantly up-regulated by the factors 9.11 ( P & lt ; 0.001 ) , 10.07 ( P & lt ; 0.001 ) and 4.08 ( P & lt ; 0.05 ) in abstinent , addicted and methadone maintained subjects , respectively relative to control group .
	manualset3
89095	6	398890	13	NULL	NULL	0	NULL	addicted subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the NR3B mRNA expression was significantly up-regulated by the factors 9.11 ( P & lt ; 0.001 ) , 10.07 ( P & lt ; 0.001 ) and 4.08 ( P & lt ; 0.05 ) in abstinent , addicted and methadone maintained subjects , respectively relative to control group .
	manualset3
89097	7	398890	13	NULL	NULL	0	NULL	methadone maintained subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the NR3B mRNA expression was significantly up-regulated by the factors 9.11 ( P & lt ; 0.001 ) , 10.07 ( P & lt ; 0.001 ) and 4.08 ( P & lt ; 0.05 ) in abstinent , addicted and methadone maintained subjects , respectively relative to control group .
	manualset3
89098	8	398890	13	NULL	NULL	0	NULL	control group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the NR3B mRNA expression was significantly up-regulated by the factors 9.11 ( P & lt ; 0.001 ) , 10.07 ( P & lt ; 0.001 ) and 4.08 ( P & lt ; 0.05 ) in abstinent , addicted and methadone maintained subjects , respectively relative to control group .
	manualset3
89100	9	398890	13	NULL	NULL	0	NULL	factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the NR3B mRNA expression was significantly up-regulated by the factors 9.11 ( P & lt ; 0.001 ) , 10.07 ( P & lt ; 0.001 ) and 4.08 ( P & lt ; 0.05 ) in abstinent , addicted and methadone maintained subjects , respectively relative to control group .
	manualset3
89225	1	398891	13	NULL	NULL	NULL	NULL	RNA content	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the RNA content ( cytophotometry ) and the total protein content ( cytophotometry and micro-interferometry ) are relatively low in the tumor cells .
	manualset3
89226	2	398891	13	NULL	NULL	0	NULL	cytophotometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the RNA content ( cytophotometry ) and the total protein content ( cytophotometry and micro-interferometry ) are relatively low in the tumor cells .
	manualset3
89227	3	398891	13	NULL	NULL	0	NULL	protein content 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the RNA content ( cytophotometry ) and the total protein content ( cytophotometry and micro-interferometry ) are relatively low in the tumor cells .
	manualset3
89228	4	398891	13	NULL	NULL	0	NULL	cytophotometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the RNA content ( cytophotometry ) and the total protein content ( cytophotometry and micro-interferometry ) are relatively low in the tumor cells .
	manualset3
89229	5	398891	13	NULL	NULL	0	NULL	micro-interferometry 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the RNA content ( cytophotometry ) and the total protein content ( cytophotometry and micro-interferometry ) are relatively low in the tumor cells .
	manualset3
89230	6	398891	13	NULL	NULL	0	NULL	tumor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the RNA content ( cytophotometry ) and the total protein content ( cytophotometry and micro-interferometry ) are relatively low in the tumor cells .
	manualset3
89231	1	398892	13	NULL	NULL	0	NULL	T-cadherin amino acid motif 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the T-cadherin amino acid motif has been well conserved through evolution in vertebrates , suggesting that T-cadherin may have biological significance in higher animals .
	manualset3
89232	2	398892	13	NULL	NULL	0	NULL	 evolution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the T-cadherin amino acid motif has been well conserved through evolution in vertebrates , suggesting that T-cadherin may have biological significance in higher animals .
	manualset3
89233	3	398892	13	NULL	NULL	0	NULL	vertebrates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the T-cadherin amino acid motif has been well conserved through evolution in vertebrates , suggesting that T-cadherin may have biological significance in higher animals .
	manualset3
89234	4	398892	13	NULL	NULL	0	NULL	T-cadherin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the T-cadherin amino acid motif has been well conserved through evolution in vertebrates , suggesting that T-cadherin may have biological significance in higher animals .
	manualset3
89235	5	398892	13	NULL	NULL	0	NULL	biological significance	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the T-cadherin amino acid motif has been well conserved through evolution in vertebrates , suggesting that T-cadherin may have biological significance in higher animals .
	manualset3
89236	6	398892	13	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the T-cadherin amino acid motif has been well conserved through evolution in vertebrates , suggesting that T-cadherin may have biological significance in higher animals .
	manualset3
89237	1	398893	13	NULL	NULL	0	NULL	X-ray cocrystal structure	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the X-ray cocrystal structure of the antithrombin-pentasaccharide complex shows that Trp49 does not contact the bound saccharide .
	manualset3
89238	2	398893	13	NULL	NULL	0	NULL	antithrombin-pentasaccharide complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the X-ray cocrystal structure of the antithrombin-pentasaccharide complex shows that Trp49 does not contact the bound saccharide .
	manualset3
89239	3	398893	13	NULL	NULL	0	NULL	Trp49	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the X-ray cocrystal structure of the antithrombin-pentasaccharide complex shows that Trp49 does not contact the bound saccharide .
	manualset3
89240	4	398893	13	NULL	NULL	0	NULL	saccharide 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the X-ray cocrystal structure of the antithrombin-pentasaccharide complex shows that Trp49 does not contact the bound saccharide .
	manualset3
89241	1	398894	13	NULL	NULL	0	NULL	future 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	( The future of the medical profession ) .
	manualset3
89242	2	398894	13	NULL	NULL	0	NULL	medical profession	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( The future of the medical profession ) .
	manualset3
89243	1	398895	13	NULL	NULL	0	NULL	agglomerates	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the agglomerates had a smaller fractal dimension ( D ( f ) = 1.28 0.08 ) ( i.e. , loosely bound ) and were found to be cytotoxic to the HaCaT cells , with a significant decrease in cell viability occurring at 25 g/mL and higher .
	manualset3
89244	2	398895	13	NULL	NULL	0	NULL	smaller fractal dimension ( D ( f ) = 1.28 0.08 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the agglomerates had a smaller fractal dimension ( D ( f ) = 1.28 0.08 ) ( i.e. , loosely bound ) and were found to be cytotoxic to the HaCaT cells , with a significant decrease in cell viability occurring at 25 g/mL and higher .
	manualset3
89245	3	398895	13	NULL	NULL	0	NULL	HaCaT cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the agglomerates had a smaller fractal dimension ( D ( f ) = 1.28 0.08 ) ( i.e. , loosely bound ) and were found to be cytotoxic to the HaCaT cells , with a significant decrease in cell viability occurring at 25 g/mL and higher .
	manualset3
89246	4	398895	13	NULL	NULL	0	NULL	cell viability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the agglomerates had a smaller fractal dimension ( D ( f ) = 1.28 0.08 ) ( i.e. , loosely bound ) and were found to be cytotoxic to the HaCaT cells , with a significant decrease in cell viability occurring at 25 g/mL and higher .
	manualset3
89247	5	398895	13	NULL	NULL	0	NULL	25 g/mL 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the agglomerates had a smaller fractal dimension ( D ( f ) = 1.28 0.08 ) ( i.e. , loosely bound ) and were found to be cytotoxic to the HaCaT cells , with a significant decrease in cell viability occurring at 25 g/mL and higher .
	manualset3
89248	1	398896	13	NULL	NULL	0	NULL	antigenic epitopes	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the antigenic epitopes of human spermatozoa , which induced antibody production , are xenogenic for the mouse , and therefore there is a possibility that there is a difference in recognized antigenic epitopes in humans as isotypic and in mice as xenogenic .
	manualset3
89249	2	398896	13	NULL	NULL	0	NULL	human spermatozoa 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the antigenic epitopes of human spermatozoa , which induced antibody production , are xenogenic for the mouse , and therefore there is a possibility that there is a difference in recognized antigenic epitopes in humans as isotypic and in mice as xenogenic .
	manualset3
89250	3	398896	13	NULL	NULL	NULL	NULL	antibody production	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the antigenic epitopes of human spermatozoa , which induced antibody production , are xenogenic for the mouse , and therefore there is a possibility that there is a difference in recognized antigenic epitopes in humans as isotypic and in mice as xenogenic .
	manualset3
89251	4	398896	13	NULL	NULL	0	NULL	mouse 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the antigenic epitopes of human spermatozoa , which induced antibody production , are xenogenic for the mouse , and therefore there is a possibility that there is a difference in recognized antigenic epitopes in humans as isotypic and in mice as xenogenic .
	manualset3
89252	5	398896	13	NULL	NULL	0	NULL	antigenic epitopes	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the antigenic epitopes of human spermatozoa , which induced antibody production , are xenogenic for the mouse , and therefore there is a possibility that there is a difference in recognized antigenic epitopes in humans as isotypic and in mice as xenogenic .
	manualset3
89253	6	398896	13	NULL	NULL	0	NULL	humans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the antigenic epitopes of human spermatozoa , which induced antibody production , are xenogenic for the mouse , and therefore there is a possibility that there is a difference in recognized antigenic epitopes in humans as isotypic and in mice as xenogenic .
	manualset3
89254	7	398896	13	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the antigenic epitopes of human spermatozoa , which induced antibody production , are xenogenic for the mouse , and therefore there is a possibility that there is a difference in recognized antigenic epitopes in humans as isotypic and in mice as xenogenic .
	manualset3
89255	1	398897	13	NULL	NULL	0	NULL	aptamer	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the aptamer does not completely block small synthetic substrate cleavage , although it does slow the rate of cleavage .
	manualset3
89256	2	398897	13	NULL	NULL	0	NULL	substrate cleavage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the aptamer does not completely block small synthetic substrate cleavage , although it does slow the rate of cleavage .
	manualset3
89257	3	398897	13	NULL	NULL	0	NULL	rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the aptamer does not completely block small synthetic substrate cleavage , although it does slow the rate of cleavage .
	manualset3
89258	4	398897	13	NULL	NULL	0	NULL	cleavage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the aptamer does not completely block small synthetic substrate cleavage , although it does slow the rate of cleavage .
	manualset3
89259	1	398898	13	NULL	NULL	0	NULL	 bursting activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the bursting activity elicited by d-amphetamine was blocked in the presence of ouabain or in the medium containing potassium-free , low sodium solutions .
	manualset3
89260	2	398898	13	NULL	NULL	0	NULL	d-amphetamine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the bursting activity elicited by d-amphetamine was blocked in the presence of ouabain or in the medium containing potassium-free , low sodium solutions .
	manualset3
89261	3	398898	13	NULL	NULL	0	NULL	ouabain	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the bursting activity elicited by d-amphetamine was blocked in the presence of ouabain or in the medium containing potassium-free , low sodium solutions .
	manualset3
89262	4	398898	13	NULL	NULL	0	NULL	medium 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the bursting activity elicited by d-amphetamine was blocked in the presence of ouabain or in the medium containing potassium-free , low sodium solutions .
	manualset3
89263	5	398898	13	NULL	NULL	0	NULL	potassium-free solutions 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the bursting activity elicited by d-amphetamine was blocked in the presence of ouabain or in the medium containing potassium-free , low sodium solutions .
	manualset3
89264	6	398898	13	NULL	NULL	0	NULL	low sodium solutions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the bursting activity elicited by d-amphetamine was blocked in the presence of ouabain or in the medium containing potassium-free , low sodium solutions .
	manualset3
89265	1	398899	13	NULL	NULL	0	NULL	 carba-analogue compound 4	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the carba-analogue compound 4 is almost ineffective .
	manualset3
89266	1	398900	13	NULL	NULL	0	NULL	cationized ferritin	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the cationized ferritin binding was preserved in the endothelial cells of the arterioles with an increased vascular permeability .
	manualset3
89267	2	398900	13	NULL	NULL	0	NULL	endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the cationized ferritin binding was preserved in the endothelial cells of the arterioles with an increased vascular permeability .
	manualset3
89268	3	398900	13	NULL	NULL	0	NULL	arterioles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the cationized ferritin binding was preserved in the endothelial cells of the arterioles with an increased vascular permeability .
	manualset3
89269	4	398900	13	NULL	NULL	0	NULL	vascular permeability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the cationized ferritin binding was preserved in the endothelial cells of the arterioles with an increased vascular permeability .
	manualset3
89270	1	398901	13	NULL	NULL	0	NULL	cell-free assay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the cell-free assay provides an incomplete representation of the assembly and regulation of the NADPH oxidase in vivo , and it has become necessary to develop methods for introducing biomolecules , such as peptides , into intact neutrophils where their effects can be investigated .
	manualset3
89271	2	398901	13	NULL	NULL	NULL	NULL	assembly 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the cell-free assay provides an incomplete representation of the assembly and regulation of the NADPH oxidase in vivo , and it has become necessary to develop methods for introducing biomolecules , such as peptides , into intact neutrophils where their effects can be investigated .
	manualset3
89272	3	398901	13	NULL	NULL	0	NULL	regulation of the NADPH oxidase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the cell-free assay provides an incomplete representation of the assembly and regulation of the NADPH oxidase in vivo , and it has become necessary to develop methods for introducing biomolecules , such as peptides , into intact neutrophils where their effects can be investigated .
	manualset3
89273	4	398901	13	NULL	NULL	0	NULL	methods 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the cell-free assay provides an incomplete representation of the assembly and regulation of the NADPH oxidase in vivo , and it has become necessary to develop methods for introducing biomolecules , such as peptides , into intact neutrophils where their effects can be investigated .
	manualset3
89274	5	398901	13	NULL	NULL	0	NULL	biomolecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the cell-free assay provides an incomplete representation of the assembly and regulation of the NADPH oxidase in vivo , and it has become necessary to develop methods for introducing biomolecules , such as peptides , into intact neutrophils where their effects can be investigated .
	manualset3
89275	6	398901	13	NULL	NULL	0	NULL	peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the cell-free assay provides an incomplete representation of the assembly and regulation of the NADPH oxidase in vivo , and it has become necessary to develop methods for introducing biomolecules , such as peptides , into intact neutrophils where their effects can be investigated .
	manualset3
89276	7	398901	13	NULL	NULL	0	NULL	neutrophils	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the cell-free assay provides an incomplete representation of the assembly and regulation of the NADPH oxidase in vivo , and it has become necessary to develop methods for introducing biomolecules , such as peptides , into intact neutrophils where their effects can be investigated .
	manualset3
89277	8	398901	13	NULL	NULL	0	NULL	effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the cell-free assay provides an incomplete representation of the assembly and regulation of the NADPH oxidase in vivo , and it has become necessary to develop methods for introducing biomolecules , such as peptides , into intact neutrophils where their effects can be investigated .
	manualset3
89278	1	398902	13	NULL	NULL	0	NULL	question	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the central question of why it took these populations approximately 100 , 000 years to disperse from Africa to other regions of the world has never been clearly resolved .
	manualset3
89279	2	398902	13	NULL	NULL	0	NULL	populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the central question of why it took these populations approximately 100 , 000 years to disperse from Africa to other regions of the world has never been clearly resolved .
	manualset3
89280	3	398902	13	NULL	NULL	0	NULL	100 , 000 years	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the central question of why it took these populations approximately 100 , 000 years to disperse from Africa to other regions of the world has never been clearly resolved .
	manualset3
89281	4	398902	13	NULL	NULL	0	NULL	Africa	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the central question of why it took these populations approximately 100 , 000 years to disperse from Africa to other regions of the world has never been clearly resolved .
	manualset3
89282	5	398902	13	NULL	NULL	NULL	NULL	regions 	GeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the central question of why it took these populations approximately 100 , 000 years to disperse from Africa to other regions of the world has never been clearly resolved .
	manualset3
89283	6	398902	13	NULL	NULL	0	NULL	 world 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the central question of why it took these populations approximately 100 , 000 years to disperse from Africa to other regions of the world has never been clearly resolved .
	manualset3
89284	1	398903	13	NULL	NULL	0	NULL	chemical preparation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the chemical preparation of scanning electron microscope ( SEM ) specimens , although adequate for low-resolution imaging of superficial detail , is not the true representation of the chemistry and composition of the sample , as extraction and aggregation artefacts as a result of dehydrating and cross-linking agents are abundant .
	manualset3
89285	2	398903	13	NULL	NULL	0	NULL	scanning electron microscope ( SEM ) specimens	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the chemical preparation of scanning electron microscope ( SEM ) specimens , although adequate for low-resolution imaging of superficial detail , is not the true representation of the chemistry and composition of the sample , as extraction and aggregation artefacts as a result of dehydrating and cross-linking agents are abundant .
	manualset3
89286	3	398903	13	NULL	NULL	0	NULL	low-resolution imaging 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the chemical preparation of scanning electron microscope ( SEM ) specimens , although adequate for low-resolution imaging of superficial detail , is not the true representation of the chemistry and composition of the sample , as extraction and aggregation artefacts as a result of dehydrating and cross-linking agents are abundant .
	manualset3
89287	4	398903	13	NULL	NULL	NULL	NULL	chemistry of the sample	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the chemical preparation of scanning electron microscope ( SEM ) specimens , although adequate for low-resolution imaging of superficial detail , is not the true representation of the chemistry and composition of the sample , as extraction and aggregation artefacts as a result of dehydrating and cross-linking agents are abundant .
	manualset3
89288	5	398903	13	NULL	NULL	0	NULL	composition of the sample	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the chemical preparation of scanning electron microscope ( SEM ) specimens , although adequate for low-resolution imaging of superficial detail , is not the true representation of the chemistry and composition of the sample , as extraction and aggregation artefacts as a result of dehydrating and cross-linking agents are abundant .
	manualset3
89289	6	398903	13	NULL	NULL	0	NULL	extraction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the chemical preparation of scanning electron microscope ( SEM ) specimens , although adequate for low-resolution imaging of superficial detail , is not the true representation of the chemistry and composition of the sample , as extraction and aggregation artefacts as a result of dehydrating and cross-linking agents are abundant .
	manualset3
89290	7	398903	13	NULL	NULL	0	NULL	aggregation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the chemical preparation of scanning electron microscope ( SEM ) specimens , although adequate for low-resolution imaging of superficial detail , is not the true representation of the chemistry and composition of the sample , as extraction and aggregation artefacts as a result of dehydrating and cross-linking agents are abundant .
	manualset3
89291	8	398903	13	NULL	NULL	0	NULL	artefacts	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the chemical preparation of scanning electron microscope ( SEM ) specimens , although adequate for low-resolution imaging of superficial detail , is not the true representation of the chemistry and composition of the sample , as extraction and aggregation artefacts as a result of dehydrating and cross-linking agents are abundant .
	manualset3
89292	9	398903	13	NULL	NULL	0	NULL	dehydrating agents 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the chemical preparation of scanning electron microscope ( SEM ) specimens , although adequate for low-resolution imaging of superficial detail , is not the true representation of the chemistry and composition of the sample , as extraction and aggregation artefacts as a result of dehydrating and cross-linking agents are abundant .
	manualset3
89293	10	398903	13	NULL	NULL	0	NULL	cross-linking agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the chemical preparation of scanning electron microscope ( SEM ) specimens , although adequate for low-resolution imaging of superficial detail , is not the true representation of the chemistry and composition of the sample , as extraction and aggregation artefacts as a result of dehydrating and cross-linking agents are abundant .
	manualset3
89294	1	398904	13	NULL	NULL	0	NULL	comparison 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the comparison of the steady-state level of the pyruvate dehydrogenase system in the presence of different substrates in various metabolic conditions provides some evidence that accumulation of acetyl-CoA and high level of NADH may promote the phosphorylation of pyruvate dehydrogenase .
	manualset3
89295	2	398904	13	NULL	NULL	0	NULL	 steady-state level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the comparison of the steady-state level of the pyruvate dehydrogenase system in the presence of different substrates in various metabolic conditions provides some evidence that accumulation of acetyl-CoA and high level of NADH may promote the phosphorylation of pyruvate dehydrogenase .
	manualset3
89296	3	398904	13	NULL	NULL	NULL	NULL	pyruvate dehydrogenase system 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the comparison of the steady-state level of the pyruvate dehydrogenase system in the presence of different substrates in various metabolic conditions provides some evidence that accumulation of acetyl-CoA and high level of NADH may promote the phosphorylation of pyruvate dehydrogenase .
	manualset3
89297	4	398904	13	NULL	NULL	0	NULL	substrates 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the comparison of the steady-state level of the pyruvate dehydrogenase system in the presence of different substrates in various metabolic conditions provides some evidence that accumulation of acetyl-CoA and high level of NADH may promote the phosphorylation of pyruvate dehydrogenase .
	manualset3
89298	5	398904	13	NULL	NULL	0	NULL	conditions 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the comparison of the steady-state level of the pyruvate dehydrogenase system in the presence of different substrates in various metabolic conditions provides some evidence that accumulation of acetyl-CoA and high level of NADH may promote the phosphorylation of pyruvate dehydrogenase .
	manualset3
89299	6	398904	13	NULL	NULL	0	NULL	evidence 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the comparison of the steady-state level of the pyruvate dehydrogenase system in the presence of different substrates in various metabolic conditions provides some evidence that accumulation of acetyl-CoA and high level of NADH may promote the phosphorylation of pyruvate dehydrogenase .
	manualset3
89300	7	398904	13	NULL	NULL	0	NULL	accumulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the comparison of the steady-state level of the pyruvate dehydrogenase system in the presence of different substrates in various metabolic conditions provides some evidence that accumulation of acetyl-CoA and high level of NADH may promote the phosphorylation of pyruvate dehydrogenase .
	manualset3
89301	8	398904	13	NULL	NULL	0	NULL	acetyl-CoA 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the comparison of the steady-state level of the pyruvate dehydrogenase system in the presence of different substrates in various metabolic conditions provides some evidence that accumulation of acetyl-CoA and high level of NADH may promote the phosphorylation of pyruvate dehydrogenase .
	manualset3
89302	9	398904	13	NULL	NULL	0	NULL	 NADH	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the comparison of the steady-state level of the pyruvate dehydrogenase system in the presence of different substrates in various metabolic conditions provides some evidence that accumulation of acetyl-CoA and high level of NADH may promote the phosphorylation of pyruvate dehydrogenase .
	manualset3
89303	10	398904	13	NULL	NULL	0	NULL	 phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the comparison of the steady-state level of the pyruvate dehydrogenase system in the presence of different substrates in various metabolic conditions provides some evidence that accumulation of acetyl-CoA and high level of NADH may promote the phosphorylation of pyruvate dehydrogenase .
	manualset3
89304	11	398904	13	NULL	NULL	0	NULL	pyruvate dehydrogenase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the comparison of the steady-state level of the pyruvate dehydrogenase system in the presence of different substrates in various metabolic conditions provides some evidence that accumulation of acetyl-CoA and high level of NADH may promote the phosphorylation of pyruvate dehydrogenase .
	manualset3
89305	1	398905	13	NULL	NULL	0	NULL	concept	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the concept of grief in children after the loss of a sibling or a parent has been accepted only recently .
	manualset3
89306	2	398905	13	NULL	NULL	0	NULL	grief	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the concept of grief in children after the loss of a sibling or a parent has been accepted only recently .
	manualset3
89307	3	398905	13	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the concept of grief in children after the loss of a sibling or a parent has been accepted only recently .
	manualset3
89308	4	398905	13	NULL	NULL	0	NULL	loss	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the concept of grief in children after the loss of a sibling or a parent has been accepted only recently .
	manualset3
89309	5	398905	13	NULL	NULL	NULL	NULL	 sibling	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the concept of grief in children after the loss of a sibling or a parent has been accepted only recently .
	manualset3
89310	6	398905	13	NULL	NULL	NULL	NULL	parent	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the concept of grief in children after the loss of a sibling or a parent has been accepted only recently .
	manualset3
89323	1	398906	13	NULL	NULL	0	NULL	conformational change	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the conformational change of BSA at pH values above pH 8 has to be taken into account .
	manualset3
89325	2	398906	13	NULL	NULL	0	NULL	BSA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the conformational change of BSA at pH values above pH 8 has to be taken into account .
	manualset3
89327	3	398906	13	NULL	NULL	NULL	NULL	pH values	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the conformational change of BSA at pH values above pH 8 has to be taken into account .
	manualset3
89328	4	398906	13	NULL	NULL	0	NULL	pH 8	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the conformational change of BSA at pH values above pH 8 has to be taken into account .
	manualset3
89337	1	398907	13	NULL	NULL	0	NULL	consequences of stigmatization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the consequences of stigmatization were class related in that the lower the class , the greater the chance that the XYY individual would spend time in the penal as well as the medical system of society .
	manualset3
89341	2	398907	13	NULL	NULL	0	NULL	 class	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the consequences of stigmatization were class related in that the lower the class , the greater the chance that the XYY individual would spend time in the penal as well as the medical system of society .
	manualset3
89343	3	398907	13	NULL	NULL	0	NULL	 XYY individual	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the consequences of stigmatization were class related in that the lower the class , the greater the chance that the XYY individual would spend time in the penal as well as the medical system of society .
	manualset3
89344	4	398907	13	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the consequences of stigmatization were class related in that the lower the class , the greater the chance that the XYY individual would spend time in the penal as well as the medical system of society .
	manualset3
89345	5	398907	13	NULL	NULL	NULL	NULL	 medical system of society	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the consequences of stigmatization were class related in that the lower the class , the greater the chance that the XYY individual would spend time in the penal as well as the medical system of society .
	manualset3
91082	6	398907	13	NULL	NULL	0	NULL	 penal system of society	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the consequences of stigmatization were class related in that the lower the class , the greater the chance that the XYY individual would spend time in the penal as well as the medical system of society .
	manualset3
89347	1	398908	13	NULL	NULL	0	NULL	efficacy of the antibiotic	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the control efficacy of the antibiotic against Phytophthora infection was somewhat less than that of metalaxyl .
	manualset3
89348	2	398908	13	NULL	NULL	0	NULL	Phytophthora infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the control efficacy of the antibiotic against Phytophthora infection was somewhat less than that of metalaxyl .
	manualset3
89349	3	398908	13	NULL	NULL	0	NULL	metalaxyl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the control efficacy of the antibiotic against Phytophthora infection was somewhat less than that of metalaxyl .
	manualset3
89350	1	398909	13	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the correlation between lethality and connectivity is relatively weak , and some highly connected proteins can be removed without noticeable phenotypic effect .
	manualset3
89351	2	398909	13	NULL	NULL	0	NULL	lethality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the correlation between lethality and connectivity is relatively weak , and some highly connected proteins can be removed without noticeable phenotypic effect .
	manualset3
89352	3	398909	13	NULL	NULL	0	NULL	connectivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the correlation between lethality and connectivity is relatively weak , and some highly connected proteins can be removed without noticeable phenotypic effect .
	manualset3
89353	4	398909	13	NULL	NULL	0	NULL	 proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the correlation between lethality and connectivity is relatively weak , and some highly connected proteins can be removed without noticeable phenotypic effect .
	manualset3
89354	5	398909	13	NULL	NULL	0	NULL	phenotypic effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the correlation between lethality and connectivity is relatively weak , and some highly connected proteins can be removed without noticeable phenotypic effect .
	manualset3
89356	1	398910	13	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the correlation between levels of TNF and PMN counts in pleural fluid of patients with parapneumonic effusion has not been previously evaluated .
	manualset3
89357	2	398910	13	NULL	NULL	0	NULL	TNF counts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the correlation between levels of TNF and PMN counts in pleural fluid of patients with parapneumonic effusion has not been previously evaluated .
	manualset3
89358	3	398910	13	NULL	NULL	0	NULL	PMN counts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the correlation between levels of TNF and PMN counts in pleural fluid of patients with parapneumonic effusion has not been previously evaluated .
	manualset3
89359	4	398910	13	NULL	NULL	0	NULL	pleural fluid	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the correlation between levels of TNF and PMN counts in pleural fluid of patients with parapneumonic effusion has not been previously evaluated .
	manualset3
89360	5	398910	13	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the correlation between levels of TNF and PMN counts in pleural fluid of patients with parapneumonic effusion has not been previously evaluated .
	manualset3
89361	6	398910	13	NULL	NULL	0	NULL	parapneumonic effusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the correlation between levels of TNF and PMN counts in pleural fluid of patients with parapneumonic effusion has not been previously evaluated .
	manualset3
89362	1	398911	13	NULL	NULL	NULL	NULL	cost	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the cost and time required performing the intracellular calcium HTS assays in the 384-well format can be prohibitive for HTS campaigns of greater than 1 x 10 ( 6 ) wells .
	manualset3
89364	2	398911	13	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the cost and time required performing the intracellular calcium HTS assays in the 384-well format can be prohibitive for HTS campaigns of greater than 1 x 10 ( 6 ) wells .
	manualset3
89365	3	398911	13	NULL	NULL	0	NULL	intracellular calcium HTS assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the cost and time required performing the intracellular calcium HTS assays in the 384-well format can be prohibitive for HTS campaigns of greater than 1 x 10 ( 6 ) wells .
	manualset3
89383	4	398911	13	NULL	NULL	0	NULL	384-well format 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the cost and time required performing the intracellular calcium HTS assays in the 384-well format can be prohibitive for HTS campaigns of greater than 1 x 10 ( 6 ) wells .
	manualset3
89387	5	398911	13	NULL	NULL	0	NULL	HTS campaigns	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the cost and time required performing the intracellular calcium HTS assays in the 384-well format can be prohibitive for HTS campaigns of greater than 1 x 10 ( 6 ) wells .
	manualset3
89388	6	398911	13	NULL	NULL	0	NULL	1 x 10 ( 6 ) wells	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the cost and time required performing the intracellular calcium HTS assays in the 384-well format can be prohibitive for HTS campaigns of greater than 1 x 10 ( 6 ) wells .
	manualset3
89390	1	398912	13	NULL	NULL	0	NULL	implementation process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The implementation process of a new model of intensive rehabilitation in a hospital setting : the development of an innovative practice within the context of integration of settings , services and treatment models ) .
	manualset3
89391	2	398912	13	NULL	NULL	NULL	NULL	a new model of intensive rehabilitation 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The implementation process of a new model of intensive rehabilitation in a hospital setting : the development of an innovative practice within the context of integration of settings , services and treatment models ) .
	manualset3
89392	3	398912	13	NULL	NULL	0	NULL	hospital setting	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( The implementation process of a new model of intensive rehabilitation in a hospital setting : the development of an innovative practice within the context of integration of settings , services and treatment models ) .
	manualset3
89393	4	398912	13	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The implementation process of a new model of intensive rehabilitation in a hospital setting : the development of an innovative practice within the context of integration of settings , services and treatment models ) .
	manualset3
89395	5	398912	13	NULL	NULL	0	NULL	innovative practice 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( The implementation process of a new model of intensive rehabilitation in a hospital setting : the development of an innovative practice within the context of integration of settings , services and treatment models ) .
	manualset3
89398	6	398912	13	NULL	NULL	NULL	NULL	integration of settings	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The implementation process of a new model of intensive rehabilitation in a hospital setting : the development of an innovative practice within the context of integration of settings , services and treatment models ) .
	manualset3
89401	7	398912	13	NULL	NULL	0	NULL	services	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( The implementation process of a new model of intensive rehabilitation in a hospital setting : the development of an innovative practice within the context of integration of settings , services and treatment models ) .
	manualset3
89402	8	398912	13	NULL	NULL	0	NULL	treatment models	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( The implementation process of a new model of intensive rehabilitation in a hospital setting : the development of an innovative practice within the context of integration of settings , services and treatment models ) .
	manualset3
89404	1	398913	13	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the critical difference between ACL and MCL is still unclear in their healing potential and cellular response .
	manualset3
89407	2	398913	13	NULL	NULL	0	NULL	ACL	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the critical difference between ACL and MCL is still unclear in their healing potential and cellular response .
	manualset3
89408	3	398913	13	NULL	NULL	0	NULL	MCL 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the critical difference between ACL and MCL is still unclear in their healing potential and cellular response .
	manualset3
89409	4	398913	13	NULL	NULL	0	NULL	healing potential	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the critical difference between ACL and MCL is still unclear in their healing potential and cellular response .
	manualset3
89410	5	398913	13	NULL	NULL	0	NULL	cellular response 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the critical difference between ACL and MCL is still unclear in their healing potential and cellular response .
	manualset3
89411	1	398914	13	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the data suggested that if health care providers provide women with information regarding their personal breast cancer risk and make a personalized recommendation for their breast cancer screening , greater compliance with screening guidelines would occur .
	manualset3
89412	2	398914	13	NULL	NULL	0	NULL	health care providers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the data suggested that if health care providers provide women with information regarding their personal breast cancer risk and make a personalized recommendation for their breast cancer screening , greater compliance with screening guidelines would occur .
	manualset3
89413	3	398914	13	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the data suggested that if health care providers provide women with information regarding their personal breast cancer risk and make a personalized recommendation for their breast cancer screening , greater compliance with screening guidelines would occur .
	manualset3
89415	4	398914	13	NULL	NULL	0	NULL	information 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the data suggested that if health care providers provide women with information regarding their personal breast cancer risk and make a personalized recommendation for their breast cancer screening , greater compliance with screening guidelines would occur .
	manualset3
89417	5	398914	13	NULL	NULL	0	NULL	personal breast cancer risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the data suggested that if health care providers provide women with information regarding their personal breast cancer risk and make a personalized recommendation for their breast cancer screening , greater compliance with screening guidelines would occur .
	manualset3
89418	6	398914	13	NULL	NULL	0	NULL	personalized recommendation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the data suggested that if health care providers provide women with information regarding their personal breast cancer risk and make a personalized recommendation for their breast cancer screening , greater compliance with screening guidelines would occur .
	manualset3
89420	7	398914	13	NULL	NULL	0	NULL	breast cancer screening 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the data suggested that if health care providers provide women with information regarding their personal breast cancer risk and make a personalized recommendation for their breast cancer screening , greater compliance with screening guidelines would occur .
	manualset3
89424	8	398914	13	NULL	NULL	0	NULL	compliance	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the data suggested that if health care providers provide women with information regarding their personal breast cancer risk and make a personalized recommendation for their breast cancer screening , greater compliance with screening guidelines would occur .
	manualset3
89425	9	398914	13	NULL	NULL	0	NULL	screening guidelines	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the data suggested that if health care providers provide women with information regarding their personal breast cancer risk and make a personalized recommendation for their breast cancer screening , greater compliance with screening guidelines would occur .
	manualset3
89426	1	398915	13	NULL	NULL	NULL	NULL	ubiquitin E3 ligases	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the dedicated ubiquitin E3 ligases targeting mitochondria for autophagy have not been revealed .
	manualset3
89427	2	398915	13	NULL	NULL	0	NULL	mitochondria	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the dedicated ubiquitin E3 ligases targeting mitochondria for autophagy have not been revealed .
	manualset3
89428	3	398915	13	NULL	NULL	0	NULL	autophagy 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the dedicated ubiquitin E3 ligases targeting mitochondria for autophagy have not been revealed .
	manualset3
89429	1	398916	13	NULL	NULL	0	NULL	detection limits	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the detection limits depend considerably on the size of the HA oligomer with larger oligomers being less sensitively detectable .
	manualset3
89431	2	398916	13	NULL	NULL	0	NULL	size	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the detection limits depend considerably on the size of the HA oligomer with larger oligomers being less sensitively detectable .
	manualset3
89433	3	398916	13	NULL	NULL	0	NULL	HA oligomer	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the detection limits depend considerably on the size of the HA oligomer with larger oligomers being less sensitively detectable .
	manualset3
89434	4	398916	13	NULL	NULL	0	NULL	oligomers	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the detection limits depend considerably on the size of the HA oligomer with larger oligomers being less sensitively detectable .
	manualset3
89437	1	398917	13	NULL	NULL	0	NULL	diagnostic accuracy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the diagnostic accuracy of individual imaging techniques is still limited .
	manualset3
89438	2	398917	13	NULL	NULL	0	NULL	individual imaging techniques	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the diagnostic accuracy of individual imaging techniques is still limited .
	manualset3
89440	1	398918	13	NULL	NULL	0	NULL	inconsistency	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the dispute about the inconsistency of data concerning the site-specific mechanism of colorectal carcinoma does exist , and more evidence about molecular events of carcinogenesis and targeted therapy needs to be collected to definitely confirm the conception .
	manualset3
89441	2	398918	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the dispute about the inconsistency of data concerning the site-specific mechanism of colorectal carcinoma does exist , and more evidence about molecular events of carcinogenesis and targeted therapy needs to be collected to definitely confirm the conception .
	manualset3
89443	3	398918	13	NULL	NULL	NULL	NULL	site-specific mechanism 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the dispute about the inconsistency of data concerning the site-specific mechanism of colorectal carcinoma does exist , and more evidence about molecular events of carcinogenesis and targeted therapy needs to be collected to definitely confirm the conception .
	manualset3
89444	4	398918	13	NULL	NULL	0	NULL	colorectal carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the dispute about the inconsistency of data concerning the site-specific mechanism of colorectal carcinoma does exist , and more evidence about molecular events of carcinogenesis and targeted therapy needs to be collected to definitely confirm the conception .
	manualset3
89447	5	398918	13	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the dispute about the inconsistency of data concerning the site-specific mechanism of colorectal carcinoma does exist , and more evidence about molecular events of carcinogenesis and targeted therapy needs to be collected to definitely confirm the conception .
	manualset3
89448	6	398918	13	NULL	NULL	0	NULL	molecular events	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the dispute about the inconsistency of data concerning the site-specific mechanism of colorectal carcinoma does exist , and more evidence about molecular events of carcinogenesis and targeted therapy needs to be collected to definitely confirm the conception .
	manualset3
89449	7	398918	13	NULL	NULL	0	NULL	carcinogenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the dispute about the inconsistency of data concerning the site-specific mechanism of colorectal carcinoma does exist , and more evidence about molecular events of carcinogenesis and targeted therapy needs to be collected to definitely confirm the conception .
	manualset3
89450	8	398918	13	NULL	NULL	0	NULL	targeted therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the dispute about the inconsistency of data concerning the site-specific mechanism of colorectal carcinoma does exist , and more evidence about molecular events of carcinogenesis and targeted therapy needs to be collected to definitely confirm the conception .
	manualset3
89451	9	398918	13	NULL	NULL	0	NULL	conception	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the dispute about the inconsistency of data concerning the site-specific mechanism of colorectal carcinoma does exist , and more evidence about molecular events of carcinogenesis and targeted therapy needs to be collected to definitely confirm the conception .
	manualset3
89455	1	398919	13	NULL	NULL	0	NULL	dissociation constant ( K ( d ) )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the dissociation constant ( K ( d ) ) for the interaction between TIAR RRM2 and the WNV 3 ' ( - ) SL RNA was 1.5 x 10 ( -8 ) , while that for TIA-1 RRM2 was 1.12 x 10 ( -7 ) .
	manualset3
89457	2	398919	13	NULL	NULL	0	NULL	 interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the dissociation constant ( K ( d ) ) for the interaction between TIAR RRM2 and the WNV 3 ' ( - ) SL RNA was 1.5 x 10 ( -8 ) , while that for TIA-1 RRM2 was 1.12 x 10 ( -7 ) .
	manualset3
89460	3	398919	13	NULL	NULL	NULL	NULL	TIAR RRM2	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the dissociation constant ( K ( d ) ) for the interaction between TIAR RRM2 and the WNV 3 ' ( - ) SL RNA was 1.5 x 10 ( -8 ) , while that for TIA-1 RRM2 was 1.12 x 10 ( -7 ) .
	manualset3
89461	4	398919	13	NULL	NULL	0	NULL	WNV 3 ' ( - ) SL RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the dissociation constant ( K ( d ) ) for the interaction between TIAR RRM2 and the WNV 3 ' ( - ) SL RNA was 1.5 x 10 ( -8 ) , while that for TIA-1 RRM2 was 1.12 x 10 ( -7 ) .
	manualset3
89463	5	398919	13	NULL	NULL	0	NULL	1.5 x 10 ( -8 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the dissociation constant ( K ( d ) ) for the interaction between TIAR RRM2 and the WNV 3 ' ( - ) SL RNA was 1.5 x 10 ( -8 ) , while that for TIA-1 RRM2 was 1.12 x 10 ( -7 ) .
	manualset3
89464	6	398919	13	NULL	NULL	NULL	NULL	TIA-1 RRM2	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the dissociation constant ( K ( d ) ) for the interaction between TIAR RRM2 and the WNV 3 ' ( - ) SL RNA was 1.5 x 10 ( -8 ) , while that for TIA-1 RRM2 was 1.12 x 10 ( -7 ) .
	manualset3
89466	7	398919	13	NULL	NULL	0	NULL	1.12 x 10 ( -7 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the dissociation constant ( K ( d ) ) for the interaction between TIAR RRM2 and the WNV 3 ' ( - ) SL RNA was 1.5 x 10 ( -8 ) , while that for TIA-1 RRM2 was 1.12 x 10 ( -7 ) .
	manualset3
89474	1	398920	13	NULL	NULL	0	NULL	H1c haplotype	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the effect is not strong , and the H1c haplotype is not involved , suggesting a mechanism that is distinct to that involved in the associated tauopathies and may be explained by the H1/H2 inversion .
	manualset3
89476	2	398920	13	NULL	NULL	0	NULL	mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the effect is not strong , and the H1c haplotype is not involved , suggesting a mechanism that is distinct to that involved in the associated tauopathies and may be explained by the H1/H2 inversion .
	manualset3
89481	3	398920	13	NULL	NULL	0	NULL	tauopathies	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the effect is not strong , and the H1c haplotype is not involved , suggesting a mechanism that is distinct to that involved in the associated tauopathies and may be explained by the H1/H2 inversion .
	manualset3
89482	4	398920	13	NULL	NULL	0	NULL	H1/H2 inversion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the effect is not strong , and the H1c haplotype is not involved , suggesting a mechanism that is distinct to that involved in the associated tauopathies and may be explained by the H1/H2 inversion .
	manualset3
89494	5	398920	13	NULL	NULL	0	NULL	effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the effect is not strong , and the H1c haplotype is not involved , suggesting a mechanism that is distinct to that involved in the associated tauopathies and may be explained by the H1/H2 inversion .
	manualset3
89487	1	398921	13	NULL	NULL	0	NULL	BMP-4 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the effect of BMP-4 on the release of VEGF by ARPE-19 cells has not been studied .
	manualset3
89488	2	398921	13	NULL	NULL	0	NULL	VEGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the effect of BMP-4 on the release of VEGF by ARPE-19 cells has not been studied .
	manualset3
89491	3	398921	13	NULL	NULL	0	NULL	ARPE-19 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the effect of BMP-4 on the release of VEGF by ARPE-19 cells has not been studied .
	manualset3
89493	4	398921	13	NULL	NULL	0	NULL	effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the effect of BMP-4 on the release of VEGF by ARPE-19 cells has not been studied .
	manualset3
89495	1	398922	13	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the effect of dialyzer reuse has never been assessed in an uncontrolled clinical practice setting .
	manualset3
89496	2	398922	13	NULL	NULL	0	NULL	dialyzer	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the effect of dialyzer reuse has never been assessed in an uncontrolled clinical practice setting .
	manualset3
89497	3	398922	13	NULL	NULL	0	NULL	clinical practice setting	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the effect of dialyzer reuse has never been assessed in an uncontrolled clinical practice setting .
	manualset3
89498	1	398923	13	NULL	NULL	0	NULL	 preoperative treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( The importance of pre - and postoperative treatment for success in plastic tubal surgery ) .
	manualset3
89499	2	398923	13	NULL	NULL	0	NULL	 postoperative treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( The importance of pre - and postoperative treatment for success in plastic tubal surgery ) .
	manualset3
89500	3	398923	13	NULL	NULL	0	NULL	 plastic tubal surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( The importance of pre - and postoperative treatment for success in plastic tubal surgery ) .
	manualset3
89501	1	398924	13	NULL	NULL	0	NULL	effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the effect of nitrogen on the synthesis of this toxin remains unclear because of the literature contradictory data .
	manualset3
89502	2	398924	13	NULL	NULL	0	NULL	nitrogen	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the effect of nitrogen on the synthesis of this toxin remains unclear because of the literature contradictory data .
	manualset3
89503	3	398924	13	NULL	NULL	0	NULL	synthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the effect of nitrogen on the synthesis of this toxin remains unclear because of the literature contradictory data .
	manualset3
89504	4	398924	13	NULL	NULL	0	NULL	 toxin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the effect of nitrogen on the synthesis of this toxin remains unclear because of the literature contradictory data .
	manualset3
89505	5	398924	13	NULL	NULL	0	NULL	literature contradictory data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the effect of nitrogen on the synthesis of this toxin remains unclear because of the literature contradictory data .
	manualset3
89506	1	398925	13	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the effect of the lindane + permethrin mixture was not significantly different than individual components of this mixture .
	manualset3
89507	2	398925	13	NULL	NULL	0	NULL	lindane + permethrin mixture	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the effect of the lindane + permethrin mixture was not significantly different than individual components of this mixture .
	manualset3
89508	3	398925	13	NULL	NULL	NULL	NULL	components	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the effect of the lindane + permethrin mixture was not significantly different than individual components of this mixture .
	manualset3
89509	4	398925	13	NULL	NULL	0	NULL	mixture	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the effect of the lindane + permethrin mixture was not significantly different than individual components of this mixture .
	manualset3
89510	1	398926	13	NULL	NULL	0	NULL	infrared laser light	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the effect of transient infrared laser light on neurotransmission in the CNS is still largely unknown .
	manualset3
89511	2	398926	13	NULL	NULL	0	NULL	neurotransmission	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the effect of transient infrared laser light on neurotransmission in the CNS is still largely unknown .
	manualset3
89512	3	398926	13	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the effect of transient infrared laser light on neurotransmission in the CNS is still largely unknown .
	manualset3
89513	4	398926	13	NULL	NULL	0	NULL	 CNS 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the effect of transient infrared laser light on neurotransmission in the CNS is still largely unknown .
	manualset3
89535	1	398927	13	NULL	NULL	0	NULL	social norms campaigns	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the efficacy of social norms campaigns has been mixed .
	manualset3
89541	2	398927	13	NULL	NULL	0	NULL	efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the efficacy of social norms campaigns has been mixed .
	manualset3
89514	1	398928	13	NULL	NULL	0	NULL	eggs 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the eggs were more resistant to the C. molmol effect than the adult snails , embryogenesis began to stop at 20 ppm and eggs were all killed at 60 & 80 ppm .
	manualset3
89515	2	398928	13	NULL	NULL	0	NULL	resistant 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the eggs were more resistant to the C. molmol effect than the adult snails , embryogenesis began to stop at 20 ppm and eggs were all killed at 60 & 80 ppm .
	manualset3
89516	3	398928	13	NULL	NULL	0	NULL	C. molmol 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the eggs were more resistant to the C. molmol effect than the adult snails , embryogenesis began to stop at 20 ppm and eggs were all killed at 60 & 80 ppm .
	manualset3
89517	4	398928	13	NULL	NULL	0	NULL	effect 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the eggs were more resistant to the C. molmol effect than the adult snails , embryogenesis began to stop at 20 ppm and eggs were all killed at 60 & 80 ppm .
	manualset3
89518	5	398928	13	NULL	NULL	0	NULL	adult snails	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the eggs were more resistant to the C. molmol effect than the adult snails , embryogenesis began to stop at 20 ppm and eggs were all killed at 60 & 80 ppm .
	manualset3
89519	6	398928	13	NULL	NULL	0	NULL	embryogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the eggs were more resistant to the C. molmol effect than the adult snails , embryogenesis began to stop at 20 ppm and eggs were all killed at 60 & 80 ppm .
	manualset3
89520	7	398928	13	NULL	NULL	0	NULL	20 ppm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the eggs were more resistant to the C. molmol effect than the adult snails , embryogenesis began to stop at 20 ppm and eggs were all killed at 60 & 80 ppm .
	manualset3
89521	8	398928	13	NULL	NULL	0	NULL	eggs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the eggs were more resistant to the C. molmol effect than the adult snails , embryogenesis began to stop at 20 ppm and eggs were all killed at 60 & 80 ppm .
	manualset3
89522	9	398928	13	NULL	NULL	0	NULL	60 & 80 ppm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the eggs were more resistant to the C. molmol effect than the adult snails , embryogenesis began to stop at 20 ppm and eggs were all killed at 60 & 80 ppm .
	manualset3
89523	1	398929	13	NULL	NULL	0	NULL	erythrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the erythrocytes tend to become saturated , and this phenomenon causes a nonlinear relationship between B-Pb and uptake and between metabolic and toxic effects and B-Pb .
	manualset3
89524	2	398929	13	NULL	NULL	0	NULL	phenomenon	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the erythrocytes tend to become saturated , and this phenomenon causes a nonlinear relationship between B-Pb and uptake and between metabolic and toxic effects and B-Pb .
	manualset3
89525	3	398929	13	NULL	NULL	0	NULL	nonlinear relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the erythrocytes tend to become saturated , and this phenomenon causes a nonlinear relationship between B-Pb and uptake and between metabolic and toxic effects and B-Pb .
	manualset3
89526	4	398929	13	NULL	NULL	NULL	NULL	B-Pb	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the erythrocytes tend to become saturated , and this phenomenon causes a nonlinear relationship between B-Pb and uptake and between metabolic and toxic effects and B-Pb .
	manualset3
89527	5	398929	13	NULL	NULL	0	NULL	uptake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the erythrocytes tend to become saturated , and this phenomenon causes a nonlinear relationship between B-Pb and uptake and between metabolic and toxic effects and B-Pb .
	manualset3
89528	6	398929	13	NULL	NULL	NULL	NULL	metabolic effects	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the erythrocytes tend to become saturated , and this phenomenon causes a nonlinear relationship between B-Pb and uptake and between metabolic and toxic effects and B-Pb .
	manualset3
89529	7	398929	13	NULL	NULL	0	NULL	toxic effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the erythrocytes tend to become saturated , and this phenomenon causes a nonlinear relationship between B-Pb and uptake and between metabolic and toxic effects and B-Pb .
	manualset3
89530	8	398929	13	NULL	NULL	0	NULL	B-Pb	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the erythrocytes tend to become saturated , and this phenomenon causes a nonlinear relationship between B-Pb and uptake and between metabolic and toxic effects and B-Pb .
	manualset3
89531	1	398930	13	NULL	NULL	0	NULL	harvest-induced selection 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the exact form of harvest-induced selection is generally unknown and the effects of harvest on trait variability remain unexplored .
	manualset3
89532	2	398930	13	NULL	NULL	0	NULL	effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the exact form of harvest-induced selection is generally unknown and the effects of harvest on trait variability remain unexplored .
	manualset3
89533	3	398930	13	NULL	NULL	NULL	NULL	harvest	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the exact form of harvest-induced selection is generally unknown and the effects of harvest on trait variability remain unexplored .
	manualset3
89534	4	398930	13	NULL	NULL	0	NULL	trait variability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the exact form of harvest-induced selection is generally unknown and the effects of harvest on trait variability remain unexplored .
	manualset3
89542	1	398931	13	NULL	NULL	0	NULL	follicles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the excess follicles formed shortly after birth did not persist into puberty and both adult rh-ActA - and vehicle-treated animals demonstrated normal fertility .
	manualset3
89543	2	398931	13	NULL	NULL	NULL	NULL	birth	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the excess follicles formed shortly after birth did not persist into puberty and both adult rh-ActA - and vehicle-treated animals demonstrated normal fertility .
	manualset3
89544	3	398931	13	NULL	NULL	NULL	NULL	puberty	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the excess follicles formed shortly after birth did not persist into puberty and both adult rh-ActA - and vehicle-treated animals demonstrated normal fertility .
	manualset3
89545	4	398931	13	NULL	NULL	0	NULL	adult rh-ActA-treated animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the excess follicles formed shortly after birth did not persist into puberty and both adult rh-ActA - and vehicle-treated animals demonstrated normal fertility .
	manualset3
89546	5	398931	13	NULL	NULL	0	NULL	vehicle-treated animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the excess follicles formed shortly after birth did not persist into puberty and both adult rh-ActA - and vehicle-treated animals demonstrated normal fertility .
	manualset3
89547	6	398931	13	NULL	NULL	0	NULL	fertility 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the excess follicles formed shortly after birth did not persist into puberty and both adult rh-ActA - and vehicle-treated animals demonstrated normal fertility .
	manualset3
89548	1	398932	13	NULL	NULL	0	NULL	Analyzing spatial-temporal dynamics	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Analyzing spatial-temporal dynamics of the ecological niche : a marten ( Martes martes ) population case study ) .
	manualset3
89549	2	398932	13	NULL	NULL	0	NULL	marten ( Martes martes ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Analyzing spatial-temporal dynamics of the ecological niche : a marten ( Martes martes ) population case study ) .
	manualset3
89550	3	398932	13	NULL	NULL	0	NULL	population case study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Analyzing spatial-temporal dynamics of the ecological niche : a marten ( Martes martes ) population case study ) .
	manualset3
90968	4	398932	13	NULL	NULL	0	NULL	 ecological niche 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Analyzing spatial-temporal dynamics of the ecological niche : a marten ( Martes martes ) population case study ) .
	manualset3
89551	1	398933	13	NULL	NULL	0	NULL	antibacterial activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( The in vitro antibacterial activity of cefozopran against clinically isolated bacteria ) .
	manualset3
89552	2	398933	13	NULL	NULL	0	NULL	cefozopran	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( The in vitro antibacterial activity of cefozopran against clinically isolated bacteria ) .
	manualset3
89553	3	398933	13	NULL	NULL	0	NULL	bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( The in vitro antibacterial activity of cefozopran against clinically isolated bacteria ) .
	manualset3
89554	1	398934	13	NULL	NULL	0	NULL	fatty acid composition	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the fatty acid composition of the brown adipose tissue , in the 3rd generation , was similar to that observed in the 1st and 2nd generation .
	manualset3
89555	2	398934	13	NULL	NULL	0	NULL	brown adipose tissue 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the fatty acid composition of the brown adipose tissue , in the 3rd generation , was similar to that observed in the 1st and 2nd generation .
	manualset3
89556	3	398934	13	NULL	NULL	0	NULL	 3rd generation	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the fatty acid composition of the brown adipose tissue , in the 3rd generation , was similar to that observed in the 1st and 2nd generation .
	manualset3
89557	4	398934	13	NULL	NULL	0	NULL	 1st generation	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the fatty acid composition of the brown adipose tissue , in the 3rd generation , was similar to that observed in the 1st and 2nd generation .
	manualset3
89558	5	398934	13	NULL	NULL	0	NULL	2nd generation	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the fatty acid composition of the brown adipose tissue , in the 3rd generation , was similar to that observed in the 1st and 2nd generation .
	manualset3
89559	1	398935	13	NULL	NULL	0	NULL	answer	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the final answer will require a clinical randomized trial in the management of carcinoma of the nasopharynx .
	manualset3
89561	3	398935	13	NULL	NULL	0	NULL	management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the final answer will require a clinical randomized trial in the management of carcinoma of the nasopharynx .
	manualset3
89562	4	398935	13	NULL	NULL	0	NULL	carcinoma of the nasopharynx	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the final answer will require a clinical randomized trial in the management of carcinoma of the nasopharynx .
	manualset3
90969	5	398935	13	NULL	NULL	0	NULL	clinical randomized trial	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the final answer will require a clinical randomized trial in the management of carcinoma of the nasopharynx .
	manualset3
89560	2	398936	13	NULL	NULL	NULL	NULL	implementation 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the implementation of hypothermia in the treatment of stroke patients is still far from routine clinical practice .
	manualset3
89570	3	398936	13	NULL	NULL	0	NULL	hypothermia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the implementation of hypothermia in the treatment of stroke patients is still far from routine clinical practice .
	manualset3
89571	4	398936	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the implementation of hypothermia in the treatment of stroke patients is still far from routine clinical practice .
	manualset3
89572	5	398936	13	NULL	NULL	0	NULL	stroke patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the implementation of hypothermia in the treatment of stroke patients is still far from routine clinical practice .
	manualset3
89573	6	398936	13	NULL	NULL	0	NULL	routine clinical practice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the implementation of hypothermia in the treatment of stroke patients is still far from routine clinical practice .
	manualset3
89574	1	398937	13	NULL	NULL	0	NULL	improvements in blood pressure 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the improvements in blood pressure and lipids demonstrated in the intervention group suggest that grapefruit should be further evaluated in the context of obesity and cardiovascular disease prevention .
	manualset3
89575	2	398937	13	NULL	NULL	0	NULL	 improvements in lipids	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the improvements in blood pressure and lipids demonstrated in the intervention group suggest that grapefruit should be further evaluated in the context of obesity and cardiovascular disease prevention .
	manualset3
89576	3	398937	13	NULL	NULL	0	NULL	intervention group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the improvements in blood pressure and lipids demonstrated in the intervention group suggest that grapefruit should be further evaluated in the context of obesity and cardiovascular disease prevention .
	manualset3
89577	4	398937	13	NULL	NULL	0	NULL	grapefruit	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the improvements in blood pressure and lipids demonstrated in the intervention group suggest that grapefruit should be further evaluated in the context of obesity and cardiovascular disease prevention .
	manualset3
89578	5	398937	13	NULL	NULL	0	NULL	obesity prevention 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the improvements in blood pressure and lipids demonstrated in the intervention group suggest that grapefruit should be further evaluated in the context of obesity and cardiovascular disease prevention .
	manualset3
89579	6	398937	13	NULL	NULL	0	NULL	cardiovascular disease prevention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the improvements in blood pressure and lipids demonstrated in the intervention group suggest that grapefruit should be further evaluated in the context of obesity and cardiovascular disease prevention .
	manualset3
89580	1	398938	13	NULL	NULL	NULL	NULL	incidence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the incidence of nutritional rickets and the incidence and prevalence of hereditary rickets in Scandinavia are unknown .
	manualset3
89581	2	398938	13	NULL	NULL	0	NULL	nutritional rickets	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the incidence of nutritional rickets and the incidence and prevalence of hereditary rickets in Scandinavia are unknown .
	manualset3
89582	3	398938	13	NULL	NULL	NULL	NULL	incidence 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the incidence of nutritional rickets and the incidence and prevalence of hereditary rickets in Scandinavia are unknown .
	manualset3
89583	4	398938	13	NULL	NULL	NULL	NULL	prevalence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the incidence of nutritional rickets and the incidence and prevalence of hereditary rickets in Scandinavia are unknown .
	manualset3
89584	5	398938	13	NULL	NULL	0	NULL	hereditary rickets	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the incidence of nutritional rickets and the incidence and prevalence of hereditary rickets in Scandinavia are unknown .
	manualset3
89585	6	398938	13	NULL	NULL	0	NULL	Scandinavia	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the incidence of nutritional rickets and the incidence and prevalence of hereditary rickets in Scandinavia are unknown .
	manualset3
89586	1	398939	13	NULL	NULL	0	NULL	influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the influence of cool storage of cat spermatozoa on subsequent in vitro embryo development and quality after IVF requires further investigation .
	manualset3
89587	2	398939	13	NULL	NULL	0	NULL	cool storage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the influence of cool storage of cat spermatozoa on subsequent in vitro embryo development and quality after IVF requires further investigation .
	manualset3
89588	3	398939	13	NULL	NULL	0	NULL	cat spermatozoa	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the influence of cool storage of cat spermatozoa on subsequent in vitro embryo development and quality after IVF requires further investigation .
	manualset3
89589	4	398939	13	NULL	NULL	0	NULL	embryo development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the influence of cool storage of cat spermatozoa on subsequent in vitro embryo development and quality after IVF requires further investigation .
	manualset3
89590	5	398939	13	NULL	NULL	0	NULL	embryo quality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the influence of cool storage of cat spermatozoa on subsequent in vitro embryo development and quality after IVF requires further investigation .
	manualset3
89591	6	398939	13	NULL	NULL	0	NULL	IVF 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the influence of cool storage of cat spermatozoa on subsequent in vitro embryo development and quality after IVF requires further investigation .
	manualset3
89592	7	398939	13	NULL	NULL	NULL	NULL	investigation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the influence of cool storage of cat spermatozoa on subsequent in vitro embryo development and quality after IVF requires further investigation .
	manualset3
89593	1	398940	13	NULL	NULL	0	NULL	 influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the influence of cultivar in the rhizosphere was the opposite to that in the phyllosphere , and the higher number and activity of E. coli O157 cells in the rhizosphere may be a consequence of them not being able to gain entry to the plant as effectively .
	manualset3
89594	2	398940	13	NULL	NULL	0	NULL	cultivar	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the influence of cultivar in the rhizosphere was the opposite to that in the phyllosphere , and the higher number and activity of E. coli O157 cells in the rhizosphere may be a consequence of them not being able to gain entry to the plant as effectively .
	manualset3
89595	3	398940	13	NULL	NULL	0	NULL	rhizosphere	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the influence of cultivar in the rhizosphere was the opposite to that in the phyllosphere , and the higher number and activity of E. coli O157 cells in the rhizosphere may be a consequence of them not being able to gain entry to the plant as effectively .
	manualset3
89596	4	398940	13	NULL	NULL	0	NULL	phyllosphere	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the influence of cultivar in the rhizosphere was the opposite to that in the phyllosphere , and the higher number and activity of E. coli O157 cells in the rhizosphere may be a consequence of them not being able to gain entry to the plant as effectively .
	manualset3
89597	5	398940	13	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the influence of cultivar in the rhizosphere was the opposite to that in the phyllosphere , and the higher number and activity of E. coli O157 cells in the rhizosphere may be a consequence of them not being able to gain entry to the plant as effectively .
	manualset3
89598	6	398940	13	NULL	NULL	0	NULL	activity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the influence of cultivar in the rhizosphere was the opposite to that in the phyllosphere , and the higher number and activity of E. coli O157 cells in the rhizosphere may be a consequence of them not being able to gain entry to the plant as effectively .
	manualset3
89599	7	398940	13	NULL	NULL	0	NULL	E. coli O157 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the influence of cultivar in the rhizosphere was the opposite to that in the phyllosphere , and the higher number and activity of E. coli O157 cells in the rhizosphere may be a consequence of them not being able to gain entry to the plant as effectively .
	manualset3
89600	8	398940	13	NULL	NULL	0	NULL	rhizosphere	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the influence of cultivar in the rhizosphere was the opposite to that in the phyllosphere , and the higher number and activity of E. coli O157 cells in the rhizosphere may be a consequence of them not being able to gain entry to the plant as effectively .
	manualset3
89601	9	398940	13	NULL	NULL	0	NULL	consequence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the influence of cultivar in the rhizosphere was the opposite to that in the phyllosphere , and the higher number and activity of E. coli O157 cells in the rhizosphere may be a consequence of them not being able to gain entry to the plant as effectively .
	manualset3
89603	10	398940	13	NULL	NULL	0	NULL	 plant	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the influence of cultivar in the rhizosphere was the opposite to that in the phyllosphere , and the higher number and activity of E. coli O157 cells in the rhizosphere may be a consequence of them not being able to gain entry to the plant as effectively .
	manualset3
90970	11	398940	13	NULL	NULL	0	NULL	entry	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the influence of cultivar in the rhizosphere was the opposite to that in the phyllosphere , and the higher number and activity of E. coli O157 cells in the rhizosphere may be a consequence of them not being able to gain entry to the plant as effectively .
	manualset3
89604	1	398941	13	NULL	NULL	0	NULL	 information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the information obtained thus far has been from only subtype B from North America and Europe , and little is known about other subtypes whose V3 amino acids differ by as much as 50 % from subtype B V3 .
	manualset3
89605	2	398941	13	NULL	NULL	0	NULL	subtype B	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the information obtained thus far has been from only subtype B from North America and Europe , and little is known about other subtypes whose V3 amino acids differ by as much as 50 % from subtype B V3 .
	manualset3
89606	3	398941	13	NULL	NULL	0	NULL	North America	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the information obtained thus far has been from only subtype B from North America and Europe , and little is known about other subtypes whose V3 amino acids differ by as much as 50 % from subtype B V3 .
	manualset3
89607	4	398941	13	NULL	NULL	0	NULL	Europe	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the information obtained thus far has been from only subtype B from North America and Europe , and little is known about other subtypes whose V3 amino acids differ by as much as 50 % from subtype B V3 .
	manualset3
89608	5	398941	13	NULL	NULL	0	NULL	subtypes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the information obtained thus far has been from only subtype B from North America and Europe , and little is known about other subtypes whose V3 amino acids differ by as much as 50 % from subtype B V3 .
	manualset3
89609	6	398941	13	NULL	NULL	0	NULL	V3 amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the information obtained thus far has been from only subtype B from North America and Europe , and little is known about other subtypes whose V3 amino acids differ by as much as 50 % from subtype B V3 .
	manualset3
89610	7	398941	13	NULL	NULL	0	NULL	50 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the information obtained thus far has been from only subtype B from North America and Europe , and little is known about other subtypes whose V3 amino acids differ by as much as 50 % from subtype B V3 .
	manualset3
89611	8	398941	13	NULL	NULL	0	NULL	subtype B V3 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the information obtained thus far has been from only subtype B from North America and Europe , and little is known about other subtypes whose V3 amino acids differ by as much as 50 % from subtype B V3 .
	manualset3
89612	1	398942	13	NULL	NULL	0	NULL	 influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The influence of different forms of coenzyme on the 4th structure of succinylized aspartate-transaminase ) .
	manualset3
89613	2	398942	13	NULL	NULL	0	NULL	coenzyme	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( The influence of different forms of coenzyme on the 4th structure of succinylized aspartate-transaminase ) .
	manualset3
89614	3	398942	13	NULL	NULL	0	NULL	4th structure	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( The influence of different forms of coenzyme on the 4th structure of succinylized aspartate-transaminase ) .
	manualset3
89615	4	398942	13	NULL	NULL	0	NULL	succinylized aspartate-transaminase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( The influence of different forms of coenzyme on the 4th structure of succinylized aspartate-transaminase ) .
	manualset3
89616	1	398943	13	NULL	NULL	0	NULL	 inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the inhibition occurred even in the absence of extracellular IPAR if the cells had been preincubated with IPAR .
	manualset3
89617	2	398943	13	NULL	NULL	NULL	NULL	extracellular IPAR	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the inhibition occurred even in the absence of extracellular IPAR if the cells had been preincubated with IPAR .
	manualset3
89618	3	398943	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the inhibition occurred even in the absence of extracellular IPAR if the cells had been preincubated with IPAR .
	manualset3
89619	4	398943	13	NULL	NULL	0	NULL	 IPAR	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the inhibition occurred even in the absence of extracellular IPAR if the cells had been preincubated with IPAR .
	manualset3
89620	1	398944	13	NULL	NULL	0	NULL	iodinated alpha 1-adrenergic antagonist HEAT	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the iodinated alpha 1-adrenergic antagonist HEAT ( ( 2-beta ( 4-hydroxyphenyl ) - ethylaminomethyl ) - tetralone ) , BE 2254 ) , a radioligand with high affinity and specificity , provides autoradiographs with a higher signal to noise ratio .
	manualset3
89621	2	398944	13	NULL	NULL	0	NULL	( 2-beta ( 4-hydroxyphenyl ) - ethylaminomethyl ) - tetralone )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the iodinated alpha 1-adrenergic antagonist HEAT ( ( 2-beta ( 4-hydroxyphenyl ) - ethylaminomethyl ) - tetralone ) , BE 2254 ) , a radioligand with high affinity and specificity , provides autoradiographs with a higher signal to noise ratio .
	manualset3
89622	3	398944	13	NULL	NULL	0	NULL	BE 2254	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the iodinated alpha 1-adrenergic antagonist HEAT ( ( 2-beta ( 4-hydroxyphenyl ) - ethylaminomethyl ) - tetralone ) , BE 2254 ) , a radioligand with high affinity and specificity , provides autoradiographs with a higher signal to noise ratio .
	manualset3
89623	4	398944	13	NULL	NULL	0	NULL	radioligand	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the iodinated alpha 1-adrenergic antagonist HEAT ( ( 2-beta ( 4-hydroxyphenyl ) - ethylaminomethyl ) - tetralone ) , BE 2254 ) , a radioligand with high affinity and specificity , provides autoradiographs with a higher signal to noise ratio .
	manualset3
89624	5	398944	13	NULL	NULL	0	NULL	affinity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the iodinated alpha 1-adrenergic antagonist HEAT ( ( 2-beta ( 4-hydroxyphenyl ) - ethylaminomethyl ) - tetralone ) , BE 2254 ) , a radioligand with high affinity and specificity , provides autoradiographs with a higher signal to noise ratio .
	manualset3
89625	6	398944	13	NULL	NULL	0	NULL	specificity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the iodinated alpha 1-adrenergic antagonist HEAT ( ( 2-beta ( 4-hydroxyphenyl ) - ethylaminomethyl ) - tetralone ) , BE 2254 ) , a radioligand with high affinity and specificity , provides autoradiographs with a higher signal to noise ratio .
	manualset3
89626	7	398944	13	NULL	NULL	0	NULL	autoradiographs 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the iodinated alpha 1-adrenergic antagonist HEAT ( ( 2-beta ( 4-hydroxyphenyl ) - ethylaminomethyl ) - tetralone ) , BE 2254 ) , a radioligand with high affinity and specificity , provides autoradiographs with a higher signal to noise ratio .
	manualset3
89627	8	398944	13	NULL	NULL	NULL	NULL	signal to noise ratio	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the iodinated alpha 1-adrenergic antagonist HEAT ( ( 2-beta ( 4-hydroxyphenyl ) - ethylaminomethyl ) - tetralone ) , BE 2254 ) , a radioligand with high affinity and specificity , provides autoradiographs with a higher signal to noise ratio .
	manualset3
89628	1	398945	13	NULL	NULL	NULL	NULL	non-invasive biomarkers	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the lack of early non-invasive biomarkers has hampered our ability to diagnose kidney diseases as early as possible , and subsequently , to initiate timely , effective , and appropriate treatment .
	manualset3
89629	2	398945	13	NULL	NULL	0	NULL	kidney diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the lack of early non-invasive biomarkers has hampered our ability to diagnose kidney diseases as early as possible , and subsequently , to initiate timely , effective , and appropriate treatment .
	manualset3
89630	3	398945	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the lack of early non-invasive biomarkers has hampered our ability to diagnose kidney diseases as early as possible , and subsequently , to initiate timely , effective , and appropriate treatment .
	manualset3
89644	1	398946	13	NULL	NULL	0	NULL	DBP	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the lower DBP could not be explained statistically by any of the variables measured .
	manualset3
89648	2	398946	13	NULL	NULL	NULL	NULL	 variables 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the lower DBP could not be explained statistically by any of the variables measured .
	manualset3
89649	1	398947	13	NULL	NULL	0	NULL	mRNA of the inhibin alpha subunit	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the mRNA of the inhibin alpha subunit was not expressed in any of these .
	manualset3
89650	1	398948	13	NULL	NULL	0	NULL	 mineral constitution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the main mineral constitution of sintered bovine bone-hydroxyapatite ( Ca10 ( PO4 ) 6 ( OH ) 2 , HAP ) seems to be too stable in vivo .
	manualset3
89651	2	398948	13	NULL	NULL	0	NULL	 bovine bone-hydroxyapatite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the main mineral constitution of sintered bovine bone-hydroxyapatite ( Ca10 ( PO4 ) 6 ( OH ) 2 , HAP ) seems to be too stable in vivo .
	manualset3
89652	3	398948	13	NULL	NULL	0	NULL	Ca10 ( PO4 ) 6 ( OH ) 2 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the main mineral constitution of sintered bovine bone-hydroxyapatite ( Ca10 ( PO4 ) 6 ( OH ) 2 , HAP ) seems to be too stable in vivo .
	manualset3
89653	4	398948	13	NULL	NULL	0	NULL	HAP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the main mineral constitution of sintered bovine bone-hydroxyapatite ( Ca10 ( PO4 ) 6 ( OH ) 2 , HAP ) seems to be too stable in vivo .
	manualset3
89654	1	398949	13	NULL	NULL	0	NULL	route of transmission 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the major route of transmission remains poorly understood .
	manualset3
89655	1	398950	13	NULL	NULL	0	NULL	penetrance 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the marked incomplete penetrance and the gender bias indicate some additional genetic and/or environmental factors to disease expression .
	manualset3
89659	2	398950	13	NULL	NULL	0	NULL	gender bias	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the marked incomplete penetrance and the gender bias indicate some additional genetic and/or environmental factors to disease expression .
	manualset3
89669	3	398950	13	NULL	NULL	0	NULL	genetic factors	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the marked incomplete penetrance and the gender bias indicate some additional genetic and/or environmental factors to disease expression .
	manualset3
89670	4	398950	13	NULL	NULL	0	NULL	environmental factors 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the marked incomplete penetrance and the gender bias indicate some additional genetic and/or environmental factors to disease expression .
	manualset3
89671	5	398950	13	NULL	NULL	0	NULL	disease expression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the marked incomplete penetrance and the gender bias indicate some additional genetic and/or environmental factors to disease expression .
	manualset3
89682	1	398951	13	NULL	NULL	0	NULL	mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the mechanism by which aspirin affect platelets other than by prostaglandin blockade is unclear .
	manualset3
89683	2	398951	13	NULL	NULL	0	NULL	aspirin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the mechanism by which aspirin affect platelets other than by prostaglandin blockade is unclear .
	manualset3
89684	3	398951	13	NULL	NULL	0	NULL	platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the mechanism by which aspirin affect platelets other than by prostaglandin blockade is unclear .
	manualset3
89685	4	398951	13	NULL	NULL	0	NULL	prostaglandin blockade	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the mechanism by which aspirin affect platelets other than by prostaglandin blockade is unclear .
	manualset3
89686	1	398952	13	NULL	NULL	0	NULL	 influence	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( The influence of estrogens upon the mitotic activity and DNA synthesis in the adrenal glands of the castrated mice ) .
	manualset3
89687	2	398952	13	NULL	NULL	0	NULL	estrogens 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( The influence of estrogens upon the mitotic activity and DNA synthesis in the adrenal glands of the castrated mice ) .
	manualset3
89688	3	398952	13	NULL	NULL	0	NULL	mitotic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( The influence of estrogens upon the mitotic activity and DNA synthesis in the adrenal glands of the castrated mice ) .
	manualset3
89689	4	398952	13	NULL	NULL	NULL	NULL	DNA synthesis	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The influence of estrogens upon the mitotic activity and DNA synthesis in the adrenal glands of the castrated mice ) .
	manualset3
89690	5	398952	13	NULL	NULL	0	NULL	adrenal glands	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( The influence of estrogens upon the mitotic activity and DNA synthesis in the adrenal glands of the castrated mice ) .
	manualset3
89691	6	398952	13	NULL	NULL	0	NULL	castrated mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( The influence of estrogens upon the mitotic activity and DNA synthesis in the adrenal glands of the castrated mice ) .
	manualset3
89692	1	398953	13	NULL	NULL	0	NULL	mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the mechanism by which gJ prevents apoptosis is not understood , and it is not known whether gJ mediates additional cellular effects .
	manualset3
89693	2	398953	13	NULL	NULL	0	NULL	gJ	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the mechanism by which gJ prevents apoptosis is not understood , and it is not known whether gJ mediates additional cellular effects .
	manualset3
89694	3	398953	13	NULL	NULL	NULL	NULL	apoptosis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the mechanism by which gJ prevents apoptosis is not understood , and it is not known whether gJ mediates additional cellular effects .
	manualset3
89695	4	398953	13	NULL	NULL	0	NULL	gJ 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the mechanism by which gJ prevents apoptosis is not understood , and it is not known whether gJ mediates additional cellular effects .
	manualset3
89696	5	398953	13	NULL	NULL	0	NULL	cellular effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the mechanism by which gJ prevents apoptosis is not understood , and it is not known whether gJ mediates additional cellular effects .
	manualset3
89697	1	398954	13	NULL	NULL	NULL	NULL	mechanisms	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the mechanisms by which TMS interferes with neural activities , especially in terms of theoretical aspects , are totally unknown .
	manualset3
89698	2	398954	13	NULL	NULL	0	NULL	TMS	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the mechanisms by which TMS interferes with neural activities , especially in terms of theoretical aspects , are totally unknown .
	manualset3
89699	3	398954	13	NULL	NULL	0	NULL	neural activities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the mechanisms by which TMS interferes with neural activities , especially in terms of theoretical aspects , are totally unknown .
	manualset3
89700	4	398954	13	NULL	NULL	NULL	NULL	theoretical aspects	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the mechanisms by which TMS interferes with neural activities , especially in terms of theoretical aspects , are totally unknown .
	manualset3
89701	1	398955	13	NULL	NULL	NULL	NULL	mechanisms	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the mechanisms by which chromosomes recognize their homologous partners are poorly understood .
	manualset3
89702	2	398955	13	NULL	NULL	0	NULL	chromosomes	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the mechanisms by which chromosomes recognize their homologous partners are poorly understood .
	manualset3
89703	3	398955	13	NULL	NULL	0	NULL	homologous partners	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the mechanisms by which chromosomes recognize their homologous partners are poorly understood .
	manualset3
89704	1	398956	13	NULL	NULL	NULL	NULL	mechanisms	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the mechanisms of interaction of these hormones in NPY neurons are largely unknown .
	manualset3
89705	2	398956	13	NULL	NULL	0	NULL	 interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the mechanisms of interaction of these hormones in NPY neurons are largely unknown .
	manualset3
89706	3	398956	13	NULL	NULL	0	NULL	hormones	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the mechanisms of interaction of these hormones in NPY neurons are largely unknown .
	manualset3
89707	4	398956	13	NULL	NULL	0	NULL	NPY neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the mechanisms of interaction of these hormones in NPY neurons are largely unknown .
	manualset3
89708	1	398957	13	NULL	NULL	0	NULL	 Hebeloma	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the monophyly of Hebeloma can not be rejected outright given ITS and nLSU-rDNA data .
	manualset3
89709	2	398957	13	NULL	NULL	0	NULL	ITS	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the monophyly of Hebeloma can not be rejected outright given ITS and nLSU-rDNA data .
	manualset3
89710	3	398957	13	NULL	NULL	0	NULL	nLSU-rDNA data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the monophyly of Hebeloma can not be rejected outright given ITS and nLSU-rDNA data .
	manualset3
90971	4	398957	13	NULL	NULL	0	NULL	monophyly	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the monophyly of Hebeloma can not be rejected outright given ITS and nLSU-rDNA data .
	manualset3
89711	1	398958	13	NULL	NULL	0	NULL	wild-type strains 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the most significant difference among the wild-type strains grown under conditions promoting capsule formation was the ability to invade fish cell lines , which was significantly higher than when the same strains were grown under conditions which did not promote capsule formation .
	manualset3
89712	2	398958	13	NULL	NULL	0	NULL	conditions 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the most significant difference among the wild-type strains grown under conditions promoting capsule formation was the ability to invade fish cell lines , which was significantly higher than when the same strains were grown under conditions which did not promote capsule formation .
	manualset3
89713	3	398958	13	NULL	NULL	0	NULL	capsule formation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the most significant difference among the wild-type strains grown under conditions promoting capsule formation was the ability to invade fish cell lines , which was significantly higher than when the same strains were grown under conditions which did not promote capsule formation .
	manualset3
89714	4	398958	13	NULL	NULL	0	NULL	fish cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the most significant difference among the wild-type strains grown under conditions promoting capsule formation was the ability to invade fish cell lines , which was significantly higher than when the same strains were grown under conditions which did not promote capsule formation .
	manualset3
89715	5	398958	13	NULL	NULL	0	NULL	 strains 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the most significant difference among the wild-type strains grown under conditions promoting capsule formation was the ability to invade fish cell lines , which was significantly higher than when the same strains were grown under conditions which did not promote capsule formation .
	manualset3
89716	6	398958	13	NULL	NULL	0	NULL	conditions	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the most significant difference among the wild-type strains grown under conditions promoting capsule formation was the ability to invade fish cell lines , which was significantly higher than when the same strains were grown under conditions which did not promote capsule formation .
	manualset3
89717	7	398958	13	NULL	NULL	0	NULL	capsule formation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the most significant difference among the wild-type strains grown under conditions promoting capsule formation was the ability to invade fish cell lines , which was significantly higher than when the same strains were grown under conditions which did not promote capsule formation .
	manualset3
89718	1	398959	13	NULL	NULL	0	NULL	influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The influence of mechanical forces and age on the remodelling of the spongy bone in lumbar vertebrae and in the neck of the femur .
	manualset3
89719	2	398959	13	NULL	NULL	NULL	NULL	mechanical forces	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The influence of mechanical forces and age on the remodelling of the spongy bone in lumbar vertebrae and in the neck of the femur .
	manualset3
89720	3	398959	13	NULL	NULL	0	NULL	age 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	( The influence of mechanical forces and age on the remodelling of the spongy bone in lumbar vertebrae and in the neck of the femur .
	manualset3
89721	4	398959	13	NULL	NULL	NULL	NULL	 spongy bone in lumbar vertebrae	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The influence of mechanical forces and age on the remodelling of the spongy bone in lumbar vertebrae and in the neck of the femur .
	manualset3
89723	6	398959	13	NULL	NULL	0	NULL	neck of the femur	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( The influence of mechanical forces and age on the remodelling of the spongy bone in lumbar vertebrae and in the neck of the femur .
	manualset3
89724	1	398960	13	NULL	NULL	NULL	NULL	new technique 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the new technique of transhepatic pancreatic vein catheterization , supplemented by determination of local hormone gradients , allows preoperative localization of even small tumors .
	manualset3
89725	2	398960	13	NULL	NULL	0	NULL	 transhepatic pancreatic vein catheterization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the new technique of transhepatic pancreatic vein catheterization , supplemented by determination of local hormone gradients , allows preoperative localization of even small tumors .
	manualset3
89726	3	398960	13	NULL	NULL	NULL	NULL	hormone gradients	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the new technique of transhepatic pancreatic vein catheterization , supplemented by determination of local hormone gradients , allows preoperative localization of even small tumors .
	manualset3
89727	4	398960	13	NULL	NULL	NULL	NULL	preoperative localization	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the new technique of transhepatic pancreatic vein catheterization , supplemented by determination of local hormone gradients , allows preoperative localization of even small tumors .
	manualset3
89728	5	398960	13	NULL	NULL	0	NULL	tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the new technique of transhepatic pancreatic vein catheterization , supplemented by determination of local hormone gradients , allows preoperative localization of even small tumors .
	manualset3
89729	1	398961	13	NULL	NULL	0	NULL	sequence homology 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the overall sequence homology among the conserved regions of RPA1 from different species is significantly lower than that observed in the corresponding beta ' - like subunits of class II and III RNA polymerase .
	manualset3
89730	2	398961	13	NULL	NULL	NULL	NULL	 conserved regions of RPA1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the overall sequence homology among the conserved regions of RPA1 from different species is significantly lower than that observed in the corresponding beta ' - like subunits of class II and III RNA polymerase .
	manualset3
89732	4	398961	13	NULL	NULL	0	NULL	species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the overall sequence homology among the conserved regions of RPA1 from different species is significantly lower than that observed in the corresponding beta ' - like subunits of class II and III RNA polymerase .
	manualset3
89733	5	398961	13	NULL	NULL	0	NULL	beta ' - like subunits of class II RNA polymerase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the overall sequence homology among the conserved regions of RPA1 from different species is significantly lower than that observed in the corresponding beta ' - like subunits of class II and III RNA polymerase .
	manualset3
89734	6	398961	13	NULL	NULL	NULL	NULL	 beta ' - like subunits of class III RNA polymerase	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the overall sequence homology among the conserved regions of RPA1 from different species is significantly lower than that observed in the corresponding beta ' - like subunits of class II and III RNA polymerase .
	manualset3
89735	1	398962	13	NULL	NULL	0	NULL	persistence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the persistence of the oral antiallergic ( anti-PCA ) effects of azelastine for 24 h ( ID50 = 3.7 mg/kg ) does not seem to be associated with its antihistaminic or antiserotonin activities .
	manualset3
89736	2	398962	13	NULL	NULL	0	NULL	oral antiallergic ( anti-PCA ) effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the persistence of the oral antiallergic ( anti-PCA ) effects of azelastine for 24 h ( ID50 = 3.7 mg/kg ) does not seem to be associated with its antihistaminic or antiserotonin activities .
	manualset3
89737	3	398962	13	NULL	NULL	0	NULL	azelastine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the persistence of the oral antiallergic ( anti-PCA ) effects of azelastine for 24 h ( ID50 = 3.7 mg/kg ) does not seem to be associated with its antihistaminic or antiserotonin activities .
	manualset3
89738	4	398962	13	NULL	NULL	0	NULL	24 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the persistence of the oral antiallergic ( anti-PCA ) effects of azelastine for 24 h ( ID50 = 3.7 mg/kg ) does not seem to be associated with its antihistaminic or antiserotonin activities .
	manualset3
89739	5	398962	13	NULL	NULL	0	NULL	ID50 = 3.7 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the persistence of the oral antiallergic ( anti-PCA ) effects of azelastine for 24 h ( ID50 = 3.7 mg/kg ) does not seem to be associated with its antihistaminic or antiserotonin activities .
	manualset3
89740	6	398962	13	NULL	NULL	0	NULL	antihistaminic activities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the persistence of the oral antiallergic ( anti-PCA ) effects of azelastine for 24 h ( ID50 = 3.7 mg/kg ) does not seem to be associated with its antihistaminic or antiserotonin activities .
	manualset3
89741	7	398962	13	NULL	NULL	0	NULL	antiserotonin activities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the persistence of the oral antiallergic ( anti-PCA ) effects of azelastine for 24 h ( ID50 = 3.7 mg/kg ) does not seem to be associated with its antihistaminic or antiserotonin activities .
	manualset3
89742	1	398963	13	NULL	NULL	NULL	NULL	position 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the position of this nucleotide change makes it highly unlikely that it could be causative for Mbius syndrome in this patient because it does not affect known splicing sequences .
	manualset3
89743	2	398963	13	NULL	NULL	0	NULL	nucleotide change	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the position of this nucleotide change makes it highly unlikely that it could be causative for Mbius syndrome in this patient because it does not affect known splicing sequences .
	manualset3
89744	3	398963	13	NULL	NULL	0	NULL	Mbius syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the position of this nucleotide change makes it highly unlikely that it could be causative for Mbius syndrome in this patient because it does not affect known splicing sequences .
	manualset3
89745	4	398963	13	NULL	NULL	NULL	NULL	patient 	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the position of this nucleotide change makes it highly unlikely that it could be causative for Mbius syndrome in this patient because it does not affect known splicing sequences .
	manualset3
89746	5	398963	13	NULL	NULL	0	NULL	splicing sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the position of this nucleotide change makes it highly unlikely that it could be causative for Mbius syndrome in this patient because it does not affect known splicing sequences .
	manualset3
89747	1	398964	13	NULL	NULL	NULL	NULL	influence	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the potential influence of neuropsychological factors on pancreatic cancer has not been investigated to date .
	manualset3
89748	2	398964	13	NULL	NULL	0	NULL	 neuropsychological factors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the potential influence of neuropsychological factors on pancreatic cancer has not been investigated to date .
	manualset3
89749	3	398964	13	NULL	NULL	0	NULL	pancreatic cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the potential influence of neuropsychological factors on pancreatic cancer has not been investigated to date .
	manualset3
89750	4	398964	13	NULL	NULL	0	NULL	date	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the potential influence of neuropsychological factors on pancreatic cancer has not been investigated to date .
	manualset3
89751	1	398965	13	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the potential risk of inducing an atrial and/or ventricular tachyarrhythmia and the consequences of lowering ventricular filling pressures and systemic vascular resistances should be born in mind ; when using this therapeutic association , the authors suggest starting treatment with low doses of dobutamine ( 5/kg/min ) and enoximone ( 0.5 - 1 mg/kg ) with hemodynamic control and steadily increasing the doses , depending on the results obtained .
	manualset3
89752	2	398965	13	NULL	NULL	0	NULL	atrial tachyarrhythmia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the potential risk of inducing an atrial and/or ventricular tachyarrhythmia and the consequences of lowering ventricular filling pressures and systemic vascular resistances should be born in mind ; when using this therapeutic association , the authors suggest starting treatment with low doses of dobutamine ( 5/kg/min ) and enoximone ( 0.5 - 1 mg/kg ) with hemodynamic control and steadily increasing the doses , depending on the results obtained .
	manualset3
89753	3	398965	13	NULL	NULL	0	NULL	ventricular tachyarrhythmia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the potential risk of inducing an atrial and/or ventricular tachyarrhythmia and the consequences of lowering ventricular filling pressures and systemic vascular resistances should be born in mind ; when using this therapeutic association , the authors suggest starting treatment with low doses of dobutamine ( 5/kg/min ) and enoximone ( 0.5 - 1 mg/kg ) with hemodynamic control and steadily increasing the doses , depending on the results obtained .
	manualset3
89754	4	398965	13	NULL	NULL	0	NULL	consequences	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the potential risk of inducing an atrial and/or ventricular tachyarrhythmia and the consequences of lowering ventricular filling pressures and systemic vascular resistances should be born in mind ; when using this therapeutic association , the authors suggest starting treatment with low doses of dobutamine ( 5/kg/min ) and enoximone ( 0.5 - 1 mg/kg ) with hemodynamic control and steadily increasing the doses , depending on the results obtained .
	manualset3
89755	5	398965	13	NULL	NULL	0	NULL	ventricular filling pressures 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the potential risk of inducing an atrial and/or ventricular tachyarrhythmia and the consequences of lowering ventricular filling pressures and systemic vascular resistances should be born in mind ; when using this therapeutic association , the authors suggest starting treatment with low doses of dobutamine ( 5/kg/min ) and enoximone ( 0.5 - 1 mg/kg ) with hemodynamic control and steadily increasing the doses , depending on the results obtained .
	manualset3
89756	6	398965	13	NULL	NULL	0	NULL	systemic vascular resistances 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the potential risk of inducing an atrial and/or ventricular tachyarrhythmia and the consequences of lowering ventricular filling pressures and systemic vascular resistances should be born in mind ; when using this therapeutic association , the authors suggest starting treatment with low doses of dobutamine ( 5/kg/min ) and enoximone ( 0.5 - 1 mg/kg ) with hemodynamic control and steadily increasing the doses , depending on the results obtained .
	manualset3
89757	7	398965	13	NULL	NULL	0	NULL	mind	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the potential risk of inducing an atrial and/or ventricular tachyarrhythmia and the consequences of lowering ventricular filling pressures and systemic vascular resistances should be born in mind ; when using this therapeutic association , the authors suggest starting treatment with low doses of dobutamine ( 5/kg/min ) and enoximone ( 0.5 - 1 mg/kg ) with hemodynamic control and steadily increasing the doses , depending on the results obtained .
	manualset3
89758	8	398965	13	NULL	NULL	0	NULL	therapeutic association	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the potential risk of inducing an atrial and/or ventricular tachyarrhythmia and the consequences of lowering ventricular filling pressures and systemic vascular resistances should be born in mind ; when using this therapeutic association , the authors suggest starting treatment with low doses of dobutamine ( 5/kg/min ) and enoximone ( 0.5 - 1 mg/kg ) with hemodynamic control and steadily increasing the doses , depending on the results obtained .
	manualset3
89759	9	398965	13	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the potential risk of inducing an atrial and/or ventricular tachyarrhythmia and the consequences of lowering ventricular filling pressures and systemic vascular resistances should be born in mind ; when using this therapeutic association , the authors suggest starting treatment with low doses of dobutamine ( 5/kg/min ) and enoximone ( 0.5 - 1 mg/kg ) with hemodynamic control and steadily increasing the doses , depending on the results obtained .
	manualset3
89760	10	398965	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the potential risk of inducing an atrial and/or ventricular tachyarrhythmia and the consequences of lowering ventricular filling pressures and systemic vascular resistances should be born in mind ; when using this therapeutic association , the authors suggest starting treatment with low doses of dobutamine ( 5/kg/min ) and enoximone ( 0.5 - 1 mg/kg ) with hemodynamic control and steadily increasing the doses , depending on the results obtained .
	manualset3
89761	11	398965	13	NULL	NULL	NULL	NULL	low doses	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the potential risk of inducing an atrial and/or ventricular tachyarrhythmia and the consequences of lowering ventricular filling pressures and systemic vascular resistances should be born in mind ; when using this therapeutic association , the authors suggest starting treatment with low doses of dobutamine ( 5/kg/min ) and enoximone ( 0.5 - 1 mg/kg ) with hemodynamic control and steadily increasing the doses , depending on the results obtained .
	manualset3
89762	12	398965	13	NULL	NULL	0	NULL	5/kg/min	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the potential risk of inducing an atrial and/or ventricular tachyarrhythmia and the consequences of lowering ventricular filling pressures and systemic vascular resistances should be born in mind ; when using this therapeutic association , the authors suggest starting treatment with low doses of dobutamine ( 5/kg/min ) and enoximone ( 0.5 - 1 mg/kg ) with hemodynamic control and steadily increasing the doses , depending on the results obtained .
	manualset3
89763	13	398965	13	NULL	NULL	0	NULL	enoximone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the potential risk of inducing an atrial and/or ventricular tachyarrhythmia and the consequences of lowering ventricular filling pressures and systemic vascular resistances should be born in mind ; when using this therapeutic association , the authors suggest starting treatment with low doses of dobutamine ( 5/kg/min ) and enoximone ( 0.5 - 1 mg/kg ) with hemodynamic control and steadily increasing the doses , depending on the results obtained .
	manualset3
89764	14	398965	13	NULL	NULL	0	NULL	0.5 - 1 mg/kg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the potential risk of inducing an atrial and/or ventricular tachyarrhythmia and the consequences of lowering ventricular filling pressures and systemic vascular resistances should be born in mind ; when using this therapeutic association , the authors suggest starting treatment with low doses of dobutamine ( 5/kg/min ) and enoximone ( 0.5 - 1 mg/kg ) with hemodynamic control and steadily increasing the doses , depending on the results obtained .
	manualset3
89765	15	398965	13	NULL	NULL	0	NULL	hemodynamic control	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the potential risk of inducing an atrial and/or ventricular tachyarrhythmia and the consequences of lowering ventricular filling pressures and systemic vascular resistances should be born in mind ; when using this therapeutic association , the authors suggest starting treatment with low doses of dobutamine ( 5/kg/min ) and enoximone ( 0.5 - 1 mg/kg ) with hemodynamic control and steadily increasing the doses , depending on the results obtained .
	manualset3
89766	16	398965	13	NULL	NULL	NULL	NULL	low doses	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the potential risk of inducing an atrial and/or ventricular tachyarrhythmia and the consequences of lowering ventricular filling pressures and systemic vascular resistances should be born in mind ; when using this therapeutic association , the authors suggest starting treatment with low doses of dobutamine ( 5/kg/min ) and enoximone ( 0.5 - 1 mg/kg ) with hemodynamic control and steadily increasing the doses , depending on the results obtained .
	manualset3
91216	17	398965	13	NULL	NULL	0	NULL	dobutamine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the potential risk of inducing an atrial and/or ventricular tachyarrhythmia and the consequences of lowering ventricular filling pressures and systemic vascular resistances should be born in mind ; when using this therapeutic association , the authors suggest starting treatment with low doses of dobutamine ( 5/kg/min ) and enoximone ( 0.5 - 1 mg/kg ) with hemodynamic control and steadily increasing the doses , depending on the results obtained .
	manualset3
89767	1	398966	13	NULL	NULL	NULL	NULL	 C18 : 3 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the presence of C18 : 3 made differences more obvious between mixtures than the presence of C18 : 1 or C18 : 2 .
	manualset3
89768	2	398966	13	NULL	NULL	0	NULL	mixtures	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the presence of C18 : 3 made differences more obvious between mixtures than the presence of C18 : 1 or C18 : 2 .
	manualset3
89769	3	398966	13	NULL	NULL	NULL	NULL	C18 : 1 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the presence of C18 : 3 made differences more obvious between mixtures than the presence of C18 : 1 or C18 : 2 .
	manualset3
89770	4	398966	13	NULL	NULL	NULL	NULL	C18 : 2 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the presence of C18 : 3 made differences more obvious between mixtures than the presence of C18 : 1 or C18 : 2 .
	manualset3
89771	1	398967	13	NULL	NULL	0	NULL	 HCO ( 3 ) ( - )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the presence of HCO ( 3 ) ( - ) / CO ( 2 ) stimulates the Cl ( - ) - transporting activity of SLC26A9 in Xenopus laevis oocytes or SLC26A9-transduced COS-7 cells .
	manualset3
89772	2	398967	13	NULL	NULL	0	NULL	CO ( 2 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the presence of HCO ( 3 ) ( - ) / CO ( 2 ) stimulates the Cl ( - ) - transporting activity of SLC26A9 in Xenopus laevis oocytes or SLC26A9-transduced COS-7 cells .
	manualset3
89773	3	398967	13	NULL	NULL	0	NULL	Cl ( - ) - transporting activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the presence of HCO ( 3 ) ( - ) / CO ( 2 ) stimulates the Cl ( - ) - transporting activity of SLC26A9 in Xenopus laevis oocytes or SLC26A9-transduced COS-7 cells .
	manualset3
89774	4	398967	13	NULL	NULL	0	NULL	SLC26A9	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the presence of HCO ( 3 ) ( - ) / CO ( 2 ) stimulates the Cl ( - ) - transporting activity of SLC26A9 in Xenopus laevis oocytes or SLC26A9-transduced COS-7 cells .
	manualset3
89775	5	398967	13	NULL	NULL	0	NULL	Xenopus laevis oocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the presence of HCO ( 3 ) ( - ) / CO ( 2 ) stimulates the Cl ( - ) - transporting activity of SLC26A9 in Xenopus laevis oocytes or SLC26A9-transduced COS-7 cells .
	manualset3
89776	6	398967	13	NULL	NULL	0	NULL	SLC26A9-transduced COS-7 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the presence of HCO ( 3 ) ( - ) / CO ( 2 ) stimulates the Cl ( - ) - transporting activity of SLC26A9 in Xenopus laevis oocytes or SLC26A9-transduced COS-7 cells .
	manualset3
89777	1	398968	13	NULL	NULL	0	NULL	radiobiological parameters	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the radiobiological parameters of the different tumors and normal tissues are typically not taken into account during dose prescription and optimization of a treatment plan or during plan evaluation .
	manualset3
89778	2	398968	13	NULL	NULL	0	NULL	 tumors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the radiobiological parameters of the different tumors and normal tissues are typically not taken into account during dose prescription and optimization of a treatment plan or during plan evaluation .
	manualset3
89779	3	398968	13	NULL	NULL	0	NULL	tissues 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the radiobiological parameters of the different tumors and normal tissues are typically not taken into account during dose prescription and optimization of a treatment plan or during plan evaluation .
	manualset3
89780	4	398968	13	NULL	NULL	0	NULL	dose prescription	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the radiobiological parameters of the different tumors and normal tissues are typically not taken into account during dose prescription and optimization of a treatment plan or during plan evaluation .
	manualset3
89781	5	398968	13	NULL	NULL	0	NULL	dose optimization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the radiobiological parameters of the different tumors and normal tissues are typically not taken into account during dose prescription and optimization of a treatment plan or during plan evaluation .
	manualset3
89782	6	398968	13	NULL	NULL	0	NULL	treatment plan	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the radiobiological parameters of the different tumors and normal tissues are typically not taken into account during dose prescription and optimization of a treatment plan or during plan evaluation .
	manualset3
89783	7	398968	13	NULL	NULL	0	NULL	plan evaluation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the radiobiological parameters of the different tumors and normal tissues are typically not taken into account during dose prescription and optimization of a treatment plan or during plan evaluation .
	manualset3
89784	1	398969	13	NULL	NULL	0	NULL	literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the recent literature indicates that radical surgery combined with maximal radiotherapy dosage and modification of the chemotherapy schedules used in children may be required to improve the prognosis for adults with Wilms ' tumor .
	manualset3
89785	2	398969	13	NULL	NULL	0	NULL	radical surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the recent literature indicates that radical surgery combined with maximal radiotherapy dosage and modification of the chemotherapy schedules used in children may be required to improve the prognosis for adults with Wilms ' tumor .
	manualset3
89786	3	398969	13	NULL	NULL	0	NULL	radiotherapy dosage	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the recent literature indicates that radical surgery combined with maximal radiotherapy dosage and modification of the chemotherapy schedules used in children may be required to improve the prognosis for adults with Wilms ' tumor .
	manualset3
89787	4	398969	13	NULL	NULL	0	NULL	chemotherapy schedules	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the recent literature indicates that radical surgery combined with maximal radiotherapy dosage and modification of the chemotherapy schedules used in children may be required to improve the prognosis for adults with Wilms ' tumor .
	manualset3
89788	5	398969	13	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the recent literature indicates that radical surgery combined with maximal radiotherapy dosage and modification of the chemotherapy schedules used in children may be required to improve the prognosis for adults with Wilms ' tumor .
	manualset3
89789	6	398969	13	NULL	NULL	0	NULL	prognosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the recent literature indicates that radical surgery combined with maximal radiotherapy dosage and modification of the chemotherapy schedules used in children may be required to improve the prognosis for adults with Wilms ' tumor .
	manualset3
89790	7	398969	13	NULL	NULL	0	NULL	adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the recent literature indicates that radical surgery combined with maximal radiotherapy dosage and modification of the chemotherapy schedules used in children may be required to improve the prognosis for adults with Wilms ' tumor .
	manualset3
89791	8	398969	13	NULL	NULL	0	NULL	Wilms ' tumor	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the recent literature indicates that radical surgery combined with maximal radiotherapy dosage and modification of the chemotherapy schedules used in children may be required to improve the prognosis for adults with Wilms ' tumor .
	manualset3
89792	1	398970	13	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the relation between these factors and arrhythmia has hitherto not been systematically explored .
	manualset3
89793	2	398970	13	NULL	NULL	0	NULL	 factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the relation between these factors and arrhythmia has hitherto not been systematically explored .
	manualset3
89794	3	398970	13	NULL	NULL	0	NULL	arrhythmia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the relation between these factors and arrhythmia has hitherto not been systematically explored .
	manualset3
89795	1	398971	13	NULL	NULL	0	NULL	 relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the relationship between digit ratio and cognition , and spatial cognition in particular , has produced mixed results .
	manualset3
89796	2	398971	13	NULL	NULL	0	NULL	 digit ratio 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the relationship between digit ratio and cognition , and spatial cognition in particular , has produced mixed results .
	manualset3
89797	3	398971	13	NULL	NULL	0	NULL	cognition	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the relationship between digit ratio and cognition , and spatial cognition in particular , has produced mixed results .
	manualset3
89798	4	398971	13	NULL	NULL	NULL	NULL	spatial cognition	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the relationship between digit ratio and cognition , and spatial cognition in particular , has produced mixed results .
	manualset3
89799	1	398972	13	NULL	NULL	0	NULL	abundance 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the relative abundance of three POMC-end products ( i.e. lys-gamma1-MSH , acetyl-alpha-MSH , and CLIP fragment ) was higher in the HD subset .
	manualset3
89800	2	398972	13	NULL	NULL	0	NULL	POMC-end products	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the relative abundance of three POMC-end products ( i.e. lys-gamma1-MSH , acetyl-alpha-MSH , and CLIP fragment ) was higher in the HD subset .
	manualset3
89801	3	398972	13	NULL	NULL	0	NULL	 lys-gamma1-MSH	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the relative abundance of three POMC-end products ( i.e. lys-gamma1-MSH , acetyl-alpha-MSH , and CLIP fragment ) was higher in the HD subset .
	manualset3
89802	4	398972	13	NULL	NULL	0	NULL	acetyl-alpha-MSH	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the relative abundance of three POMC-end products ( i.e. lys-gamma1-MSH , acetyl-alpha-MSH , and CLIP fragment ) was higher in the HD subset .
	manualset3
89803	5	398972	13	NULL	NULL	0	NULL	CLIP fragment	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the relative abundance of three POMC-end products ( i.e. lys-gamma1-MSH , acetyl-alpha-MSH , and CLIP fragment ) was higher in the HD subset .
	manualset3
89804	6	398972	13	NULL	NULL	NULL	NULL	HD subset	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the relative abundance of three POMC-end products ( i.e. lys-gamma1-MSH , acetyl-alpha-MSH , and CLIP fragment ) was higher in the HD subset .
	manualset3
89805	1	398973	13	NULL	NULL	0	NULL	peroxisomal import experiment 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the results of an in vitro peroxisomal import experiment showed that the mutation of L9P , L13P , V17P , and A20P caused loss of the PTS function .
	manualset3
89806	2	398973	13	NULL	NULL	0	NULL	mutation of L9P 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the results of an in vitro peroxisomal import experiment showed that the mutation of L9P , L13P , V17P , and A20P caused loss of the PTS function .
	manualset3
89807	3	398973	13	NULL	NULL	0	NULL	mutation of  L13P	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the results of an in vitro peroxisomal import experiment showed that the mutation of L9P , L13P , V17P , and A20P caused loss of the PTS function .
	manualset3
89808	4	398973	13	NULL	NULL	0	NULL	mutation of  V17P	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the results of an in vitro peroxisomal import experiment showed that the mutation of L9P , L13P , V17P , and A20P caused loss of the PTS function .
	manualset3
89809	5	398973	13	NULL	NULL	0	NULL	 mutation of A20P	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the results of an in vitro peroxisomal import experiment showed that the mutation of L9P , L13P , V17P , and A20P caused loss of the PTS function .
	manualset3
89810	6	398973	13	NULL	NULL	0	NULL	PTS function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the results of an in vitro peroxisomal import experiment showed that the mutation of L9P , L13P , V17P , and A20P caused loss of the PTS function .
	manualset3
89811	1	398974	13	NULL	NULL	0	NULL	OCT-4 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the role of the OCT-4 protein in seminomas has not been clarified .
	manualset3
89812	2	398974	13	NULL	NULL	0	NULL	seminomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the role of the OCT-4 protein in seminomas has not been clarified .
	manualset3
89813	3	398974	13	NULL	NULL	0	NULL	 role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the role of the OCT-4 protein in seminomas has not been clarified .
	manualset3
89814	1	398975	13	NULL	NULL	0	NULL	role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the role that these animals play in the transmission cycle of the Leishmania spp .
	manualset3
89815	2	398975	13	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the role that these animals play in the transmission cycle of the Leishmania spp .
	manualset3
89816	3	398975	13	NULL	NULL	NULL	NULL	transmission cycle	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the role that these animals play in the transmission cycle of the Leishmania spp .
	manualset3
89817	4	398975	13	NULL	NULL	0	NULL	Leishmania spp	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the role that these animals play in the transmission cycle of the Leishmania spp .
	manualset3
89818	1	398976	13	NULL	NULL	0	NULL	mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( The mechanism of glucan-induced agglutination of Actinomyces viscosus ( author 's transl ) ) .
	manualset3
89819	2	398976	13	NULL	NULL	NULL	NULL	glucan-induced agglutination	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The mechanism of glucan-induced agglutination of Actinomyces viscosus ( author 's transl ) ) .
	manualset3
89820	3	398976	13	NULL	NULL	0	NULL	Actinomyces viscosus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( The mechanism of glucan-induced agglutination of Actinomyces viscosus ( author 's transl ) ) .
	manualset3
89821	4	398976	13	NULL	NULL	0	NULL	 author 's	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( The mechanism of glucan-induced agglutination of Actinomyces viscosus ( author 's transl ) ) .
	manualset3
89822	1	398977	13	NULL	NULL	0	NULL	treatment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the same treatment decreased the amount of 4-methylthio-3-butenylisothiocyanate ( MTBITC ) , a major isothiocyanate in radish sprout and the activity of myrosinase , an enzyme related to produce isothiocyanates .
	manualset3
89823	2	398977	13	NULL	NULL	0	NULL	4-methylthio-3-butenylisothiocyanate ( MTBITC )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the same treatment decreased the amount of 4-methylthio-3-butenylisothiocyanate ( MTBITC ) , a major isothiocyanate in radish sprout and the activity of myrosinase , an enzyme related to produce isothiocyanates .
	manualset3
89824	3	398977	13	NULL	NULL	0	NULL	amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the same treatment decreased the amount of 4-methylthio-3-butenylisothiocyanate ( MTBITC ) , a major isothiocyanate in radish sprout and the activity of myrosinase , an enzyme related to produce isothiocyanates .
	manualset3
89825	4	398977	13	NULL	NULL	NULL	NULL	 a major isothiocyanate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the same treatment decreased the amount of 4-methylthio-3-butenylisothiocyanate ( MTBITC ) , a major isothiocyanate in radish sprout and the activity of myrosinase , an enzyme related to produce isothiocyanates .
	manualset3
89826	5	398977	13	NULL	NULL	0	NULL	radish sprout 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the same treatment decreased the amount of 4-methylthio-3-butenylisothiocyanate ( MTBITC ) , a major isothiocyanate in radish sprout and the activity of myrosinase , an enzyme related to produce isothiocyanates .
	manualset3
89827	6	398977	13	NULL	NULL	0	NULL	activity of myrosinase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the same treatment decreased the amount of 4-methylthio-3-butenylisothiocyanate ( MTBITC ) , a major isothiocyanate in radish sprout and the activity of myrosinase , an enzyme related to produce isothiocyanates .
	manualset3
89828	7	398977	13	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the same treatment decreased the amount of 4-methylthio-3-butenylisothiocyanate ( MTBITC ) , a major isothiocyanate in radish sprout and the activity of myrosinase , an enzyme related to produce isothiocyanates .
	manualset3
89829	8	398977	13	NULL	NULL	0	NULL	isothiocyanates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the same treatment decreased the amount of 4-methylthio-3-butenylisothiocyanate ( MTBITC ) , a major isothiocyanate in radish sprout and the activity of myrosinase , an enzyme related to produce isothiocyanates .
	manualset3
89830	1	398978	13	NULL	NULL	0	NULL	scale shift 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the scale shift was similar between the LRCpH and the CIpH .
	manualset3
89831	2	398978	13	NULL	NULL	0	NULL	LRCpH	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the scale shift was similar between the LRCpH and the CIpH .
	manualset3
89832	3	398978	13	NULL	NULL	0	NULL	CIpH	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the scale shift was similar between the LRCpH and the CIpH .
	manualset3
89833	1	398979	13	NULL	NULL	NULL	NULL	severe cases	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the severe cases and those occurring in high risk patient must be treated ( ciprofloxacin or ceftriaxone ) .
	manualset3
89834	2	398979	13	NULL	NULL	NULL	NULL	high risk patient 	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the severe cases and those occurring in high risk patient must be treated ( ciprofloxacin or ceftriaxone ) .
	manualset3
89835	3	398979	13	NULL	NULL	0	NULL	ciprofloxacin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the severe cases and those occurring in high risk patient must be treated ( ciprofloxacin or ceftriaxone ) .
	manualset3
89836	4	398979	13	NULL	NULL	0	NULL	ceftriaxone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the severe cases and those occurring in high risk patient must be treated ( ciprofloxacin or ceftriaxone ) .
	manualset3
89837	1	398980	13	NULL	NULL	0	NULL	signal intensities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the signal intensities for IL-1mRNA and protein in the epithelium were significantly decreased after marsupialization which relived intracystic pressure .
	manualset3
89838	2	398980	13	NULL	NULL	0	NULL	IL-1mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the signal intensities for IL-1mRNA and protein in the epithelium were significantly decreased after marsupialization which relived intracystic pressure .
	manualset3
89839	3	398980	13	NULL	NULL	0	NULL	 IL-1 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the signal intensities for IL-1mRNA and protein in the epithelium were significantly decreased after marsupialization which relived intracystic pressure .
	manualset3
89840	4	398980	13	NULL	NULL	0	NULL	epithelium	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the signal intensities for IL-1mRNA and protein in the epithelium were significantly decreased after marsupialization which relived intracystic pressure .
	manualset3
89841	5	398980	13	NULL	NULL	0	NULL	marsupialization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the signal intensities for IL-1mRNA and protein in the epithelium were significantly decreased after marsupialization which relived intracystic pressure .
	manualset3
89842	6	398980	13	NULL	NULL	0	NULL	intracystic pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the signal intensities for IL-1mRNA and protein in the epithelium were significantly decreased after marsupialization which relived intracystic pressure .
	manualset3
89843	1	398981	13	NULL	NULL	NULL	NULL	CNS sites	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the specific CNS sites where ANG II inhibits baroreflexes are not completely understood .
	manualset3
89844	2	398981	13	NULL	NULL	0	NULL	ANG II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the specific CNS sites where ANG II inhibits baroreflexes are not completely understood .
	manualset3
89845	3	398981	13	NULL	NULL	0	NULL	baroreflexes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the specific CNS sites where ANG II inhibits baroreflexes are not completely understood .
	manualset3
89932	1	398982	13	NULL	NULL	0	NULL	role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the specific role of sPLA ( 2 ) - IIA in phosgene-induced acute lung injury remains unidentified .
	manualset3
89933	2	398982	13	NULL	NULL	0	NULL	sPLA ( 2 ) - IIA 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the specific role of sPLA ( 2 ) - IIA in phosgene-induced acute lung injury remains unidentified .
	manualset3
89934	3	398982	13	NULL	NULL	0	NULL	phosgene-induced acute lung injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the specific role of sPLA ( 2 ) - IIA in phosgene-induced acute lung injury remains unidentified .
	manualset3
89935	1	398983	13	NULL	NULL	NULL	NULL	 surface area of rough endoplasmic reticulum per unit volume 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the surface area of rough endoplasmic reticulum per unit volume of the supraoptic nucleus cell did differ significantly between the two age groups over the course of the experiment .
	manualset3
89936	2	398983	13	NULL	NULL	0	NULL	 supraoptic nucleus cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the surface area of rough endoplasmic reticulum per unit volume of the supraoptic nucleus cell did differ significantly between the two age groups over the course of the experiment .
	manualset3
89941	3	398983	13	NULL	NULL	0	NULL	two age groups 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the surface area of rough endoplasmic reticulum per unit volume of the supraoptic nucleus cell did differ significantly between the two age groups over the course of the experiment .
	manualset3
89942	4	398983	13	NULL	NULL	0	NULL	course	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the surface area of rough endoplasmic reticulum per unit volume of the supraoptic nucleus cell did differ significantly between the two age groups over the course of the experiment .
	manualset3
89943	5	398983	13	NULL	NULL	0	NULL	experiment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the surface area of rough endoplasmic reticulum per unit volume of the supraoptic nucleus cell did differ significantly between the two age groups over the course of the experiment .
	manualset3
89944	1	398984	13	NULL	NULL	0	NULL	medico-social problem	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( The medico-social problem in recovery from poliomyelitis ) .
	manualset3
89945	2	398984	13	NULL	NULL	0	NULL	 recovery	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( The medico-social problem in recovery from poliomyelitis ) .
	manualset3
89946	3	398984	13	NULL	NULL	0	NULL	poliomyelitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( The medico-social problem in recovery from poliomyelitis ) .
	manualset3
89947	1	398985	13	NULL	NULL	0	NULL	 time constant	Unit												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the time constant of recovery of Raw from MCh constriction was increased from control ( 40 + / - 3 s ) to 57 + / - 10 s after bradykinin infusion ( P = 0.03 ) .
	manualset3
89948	2	398985	13	NULL	NULL	0	NULL	recovery of Raw 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the time constant of recovery of Raw from MCh constriction was increased from control ( 40 + / - 3 s ) to 57 + / - 10 s after bradykinin infusion ( P = 0.03 ) .
	manualset3
89949	3	398985	13	NULL	NULL	0	NULL	MCh constriction 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the time constant of recovery of Raw from MCh constriction was increased from control ( 40 + / - 3 s ) to 57 + / - 10 s after bradykinin infusion ( P = 0.03 ) .
	manualset3
89950	4	398985	13	NULL	NULL	0	NULL	control ( 40 + / - 3 s ) to 57 + / - 10 s	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the time constant of recovery of Raw from MCh constriction was increased from control ( 40 + / - 3 s ) to 57 + / - 10 s after bradykinin infusion ( P = 0.03 ) .
	manualset3
89951	5	398985	13	NULL	NULL	0	NULL	bradykinin infusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the time constant of recovery of Raw from MCh constriction was increased from control ( 40 + / - 3 s ) to 57 + / - 10 s after bradykinin infusion ( P = 0.03 ) .
	manualset3
89952	6	398985	13	NULL	NULL	0	NULL	P = 0.03 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the time constant of recovery of Raw from MCh constriction was increased from control ( 40 + / - 3 s ) to 57 + / - 10 s after bradykinin infusion ( P = 0.03 ) .
	manualset3
89953	1	398986	13	NULL	NULL	0	NULL	tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the tumors were negative for synaptophysin and neurofilament proteins , unlike most islet cell tumors .
	manualset3
89954	2	398986	13	NULL	NULL	0	NULL	synaptophysin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the tumors were negative for synaptophysin and neurofilament proteins , unlike most islet cell tumors .
	manualset3
89955	3	398986	13	NULL	NULL	0	NULL	neurofilament proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the tumors were negative for synaptophysin and neurofilament proteins , unlike most islet cell tumors .
	manualset3
89956	4	398986	13	NULL	NULL	0	NULL	islet cell tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the tumors were negative for synaptophysin and neurofilament proteins , unlike most islet cell tumors .
	manualset3
89957	1	398987	13	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the two extended wear groups did not differ significantly ( P ) 0.2 .
	manualset3
89958	2	398987	13	NULL	NULL	NULL	NULL	extended wear groups	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the two extended wear groups did not differ significantly ( P ) 0.2 .
	manualset3
89959	3	398987	13	NULL	NULL	0	NULL	( P ) 0.2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the two extended wear groups did not differ significantly ( P ) 0.2 .
	manualset3
89960	1	398988	13	NULL	NULL	NULL	NULL	 vertical concentration distributions	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the vertical concentration distributions of soluble copper seem not affected much by the variation of sediment concentrations .
	manualset3
89961	2	398988	13	NULL	NULL	NULL	NULL	soluble copper	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the vertical concentration distributions of soluble copper seem not affected much by the variation of sediment concentrations .
	manualset3
89962	3	398988	13	NULL	NULL	0	NULL	variation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the vertical concentration distributions of soluble copper seem not affected much by the variation of sediment concentrations .
	manualset3
89963	4	398988	13	NULL	NULL	0	NULL	sediment concentrations 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the vertical concentration distributions of soluble copper seem not affected much by the variation of sediment concentrations .
	manualset3
89964	1	398989	13	NULL	NULL	0	NULL	volume	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the volume reduction compared with equivalent BNR systems with SSTs will not be large ( 40-60 % ) , but the cost of the membranes can be offset against sludge thickening and stabilisation costs .
	manualset3
89965	2	398989	13	NULL	NULL	0	NULL	 reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the volume reduction compared with equivalent BNR systems with SSTs will not be large ( 40-60 % ) , but the cost of the membranes can be offset against sludge thickening and stabilisation costs .
	manualset3
89966	3	398989	13	NULL	NULL	0	NULL	BNR systems	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the volume reduction compared with equivalent BNR systems with SSTs will not be large ( 40-60 % ) , but the cost of the membranes can be offset against sludge thickening and stabilisation costs .
	manualset3
89967	4	398989	13	NULL	NULL	0	NULL	SSTs	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the volume reduction compared with equivalent BNR systems with SSTs will not be large ( 40-60 % ) , but the cost of the membranes can be offset against sludge thickening and stabilisation costs .
	manualset3
89968	5	398989	13	NULL	NULL	0	NULL	large ( 40-60 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the volume reduction compared with equivalent BNR systems with SSTs will not be large ( 40-60 % ) , but the cost of the membranes can be offset against sludge thickening and stabilisation costs .
	manualset3
89969	6	398989	13	NULL	NULL	0	NULL	cost	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the volume reduction compared with equivalent BNR systems with SSTs will not be large ( 40-60 % ) , but the cost of the membranes can be offset against sludge thickening and stabilisation costs .
	manualset3
89970	7	398989	13	NULL	NULL	0	NULL	 membranes 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the volume reduction compared with equivalent BNR systems with SSTs will not be large ( 40-60 % ) , but the cost of the membranes can be offset against sludge thickening and stabilisation costs .
	manualset3
89971	8	398989	13	NULL	NULL	0	NULL	sludge thickening	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the volume reduction compared with equivalent BNR systems with SSTs will not be large ( 40-60 % ) , but the cost of the membranes can be offset against sludge thickening and stabilisation costs .
	manualset3
89972	9	398989	13	NULL	NULL	0	NULL	stabilisation costs 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the volume reduction compared with equivalent BNR systems with SSTs will not be large ( 40-60 % ) , but the cost of the membranes can be offset against sludge thickening and stabilisation costs .
	manualset3
89973	1	398990	13	NULL	NULL	NULL	NULL	xenogeneic CDRs 	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the xenogeneic CDRs of the humanized antibodies may evoke anti-idiotypic ( anti-Id ) response in patients .
	manualset3
89974	2	398990	13	NULL	NULL	NULL	NULL	humanized antibodies	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , the xenogeneic CDRs of the humanized antibodies may evoke anti-idiotypic ( anti-Id ) response in patients .
	manualset3
89975	3	398990	13	NULL	NULL	0	NULL	anti-idiotypic ( anti-Id ) response 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the xenogeneic CDRs of the humanized antibodies may evoke anti-idiotypic ( anti-Id ) response in patients .
	manualset3
89976	4	398990	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the xenogeneic CDRs of the humanized antibodies may evoke anti-idiotypic ( anti-Id ) response in patients .
	manualset3
89977	1	398991	13	NULL	NULL	0	NULL	rehabilitation training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The need for organized advanced rehabilitation training for handicapped adults as a condition of occupational success ) .
	manualset3
89978	2	398991	13	NULL	NULL	NULL	NULL	handicapped adults	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The need for organized advanced rehabilitation training for handicapped adults as a condition of occupational success ) .
	manualset3
89979	3	398991	13	NULL	NULL	0	NULL	condition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The need for organized advanced rehabilitation training for handicapped adults as a condition of occupational success ) .
	manualset3
89980	4	398991	13	NULL	NULL	NULL	NULL	occupational success	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The need for organized advanced rehabilitation training for handicapped adults as a condition of occupational success ) .
	manualset3
89981	1	398992	13	NULL	NULL	0	NULL	differences 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there are no significant differences between scutellarin-treated group and S. miltiorrhiza-treated group ( P & gt ; 0.05 ) .
	manualset3
89982	2	398992	13	NULL	NULL	0	NULL	 scutellarin-treated group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there are no significant differences between scutellarin-treated group and S. miltiorrhiza-treated group ( P & gt ; 0.05 ) .
	manualset3
89983	3	398992	13	NULL	NULL	0	NULL	 S. miltiorrhiza-treated group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there are no significant differences between scutellarin-treated group and S. miltiorrhiza-treated group ( P & gt ; 0.05 ) .
	manualset3
89984	4	398992	13	NULL	NULL	0	NULL	P & gt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there are no significant differences between scutellarin-treated group and S. miltiorrhiza-treated group ( P & gt ; 0.05 ) .
	manualset3
89985	1	398993	13	NULL	NULL	NULL	NULL	 indication	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , there has been some indication that cue integration may be affected by characteristics of the visual stimulus .
	manualset3
89986	2	398993	13	NULL	NULL	NULL	NULL	cue integration	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , there has been some indication that cue integration may be affected by characteristics of the visual stimulus .
	manualset3
89987	3	398993	13	NULL	NULL	NULL	NULL	visual stimulus 	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , there has been some indication that cue integration may be affected by characteristics of the visual stimulus .
	manualset3
89988	1	398994	13	NULL	NULL	0	NULL	 lack	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there is a lack of data on tumors , regarding the relationship between N-myc gene amplification and proliferation activity .
	manualset3
89989	2	398994	13	NULL	NULL	0	NULL	data on tumors	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there is a lack of data on tumors , regarding the relationship between N-myc gene amplification and proliferation activity .
	manualset3
89990	3	398994	13	NULL	NULL	0	NULL	relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there is a lack of data on tumors , regarding the relationship between N-myc gene amplification and proliferation activity .
	manualset3
89991	4	398994	13	NULL	NULL	0	NULL	 N-myc gene amplification	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there is a lack of data on tumors , regarding the relationship between N-myc gene amplification and proliferation activity .
	manualset3
89992	5	398994	13	NULL	NULL	0	NULL	 proliferation activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there is a lack of data on tumors , regarding the relationship between N-myc gene amplification and proliferation activity .
	manualset3
89993	1	398995	13	NULL	NULL	0	NULL	stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there is a possibility that long-term stimulation of neurogenesis might exhaust the proliferation potentials of neuronal progenitors .
	manualset3
89994	2	398995	13	NULL	NULL	0	NULL	neurogenesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there is a possibility that long-term stimulation of neurogenesis might exhaust the proliferation potentials of neuronal progenitors .
	manualset3
89995	3	398995	13	NULL	NULL	0	NULL	 proliferation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there is a possibility that long-term stimulation of neurogenesis might exhaust the proliferation potentials of neuronal progenitors .
	manualset3
89996	4	398995	13	NULL	NULL	NULL	NULL	neuronal progenitors 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , there is a possibility that long-term stimulation of neurogenesis might exhaust the proliferation potentials of neuronal progenitors .
	manualset3
89997	1	398996	13	NULL	NULL	0	NULL	documentation	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there is no documentation that systematic screening will have a positive effect on morbidity and mortality , owing to the lack of randomised clinical trials .
	manualset3
89998	2	398996	13	NULL	NULL	0	NULL	systematic screening 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there is no documentation that systematic screening will have a positive effect on morbidity and mortality , owing to the lack of randomised clinical trials .
	manualset3
89999	3	398996	13	NULL	NULL	0	NULL	effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there is no documentation that systematic screening will have a positive effect on morbidity and mortality , owing to the lack of randomised clinical trials .
	manualset3
90000	4	398996	13	NULL	NULL	0	NULL	morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there is no documentation that systematic screening will have a positive effect on morbidity and mortality , owing to the lack of randomised clinical trials .
	manualset3
90001	5	398996	13	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there is no documentation that systematic screening will have a positive effect on morbidity and mortality , owing to the lack of randomised clinical trials .
	manualset3
90002	6	398996	13	NULL	NULL	0	NULL	randomised clinical trials	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there is no documentation that systematic screening will have a positive effect on morbidity and mortality , owing to the lack of randomised clinical trials .
	manualset3
90003	1	398997	13	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there is no evidence that initiation of treatment , or increases in dose of opioids or sedatives , is associated with precipitation of death .
	manualset3
90004	2	398997	13	NULL	NULL	0	NULL	initiation of treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there is no evidence that initiation of treatment , or increases in dose of opioids or sedatives , is associated with precipitation of death .
	manualset3
90005	3	398997	13	NULL	NULL	0	NULL	dose of opioids 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there is no evidence that initiation of treatment , or increases in dose of opioids or sedatives , is associated with precipitation of death .
	manualset3
90006	4	398997	13	NULL	NULL	0	NULL	dose of sedatives	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there is no evidence that initiation of treatment , or increases in dose of opioids or sedatives , is associated with precipitation of death .
	manualset3
90007	5	398997	13	NULL	NULL	0	NULL	precipitation of death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there is no evidence that initiation of treatment , or increases in dose of opioids or sedatives , is associated with precipitation of death .
	manualset3
90009	1	398998	13	NULL	NULL	0	NULL	influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there is no mention of the influence of hemoglobinopathy on the ZPP test value .
	manualset3
90010	2	398998	13	NULL	NULL	0	NULL	hemoglobinopathy 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there is no mention of the influence of hemoglobinopathy on the ZPP test value .
	manualset3
90011	3	398998	13	NULL	NULL	0	NULL	ZPP test value	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there is no mention of the influence of hemoglobinopathy on the ZPP test value .
	manualset3
90012	1	398999	13	NULL	NULL	0	NULL	trend	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there was a trend for antigen-specific proliferative responses of peripheral blood mononuclear cells ( PBMC ) from booster vaccinates to be reduced compared to responses of PBMC from single vaccinates .
	manualset3
90013	2	398999	13	NULL	NULL	0	NULL	antigen-specific proliferative responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there was a trend for antigen-specific proliferative responses of peripheral blood mononuclear cells ( PBMC ) from booster vaccinates to be reduced compared to responses of PBMC from single vaccinates .
	manualset3
90014	3	398999	13	NULL	NULL	0	NULL	peripheral blood mononuclear cells ( PBMC )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there was a trend for antigen-specific proliferative responses of peripheral blood mononuclear cells ( PBMC ) from booster vaccinates to be reduced compared to responses of PBMC from single vaccinates .
	manualset3
90015	4	398999	13	NULL	NULL	0	NULL	booster vaccinates 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there was a trend for antigen-specific proliferative responses of peripheral blood mononuclear cells ( PBMC ) from booster vaccinates to be reduced compared to responses of PBMC from single vaccinates .
	manualset3
90016	5	398999	13	NULL	NULL	0	NULL	responses 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there was a trend for antigen-specific proliferative responses of peripheral blood mononuclear cells ( PBMC ) from booster vaccinates to be reduced compared to responses of PBMC from single vaccinates .
	manualset3
90017	6	398999	13	NULL	NULL	0	NULL	PBMC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there was a trend for antigen-specific proliferative responses of peripheral blood mononuclear cells ( PBMC ) from booster vaccinates to be reduced compared to responses of PBMC from single vaccinates .
	manualset3
90018	7	398999	13	NULL	NULL	0	NULL	single vaccinates	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there was a trend for antigen-specific proliferative responses of peripheral blood mononuclear cells ( PBMC ) from booster vaccinates to be reduced compared to responses of PBMC from single vaccinates .
	manualset3
90019	1	399000	13	NULL	NULL	0	NULL	correlation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there was no correlation between the colony-forming efficiency and the initial number of peripheral platelets or bone marrow megakaryocytes that contained growth-promoting factor .
	manualset3
90020	2	399000	13	NULL	NULL	0	NULL	colony-forming efficiency	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there was no correlation between the colony-forming efficiency and the initial number of peripheral platelets or bone marrow megakaryocytes that contained growth-promoting factor .
	manualset3
90021	3	399000	13	NULL	NULL	NULL	NULL	 initial number	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , there was no correlation between the colony-forming efficiency and the initial number of peripheral platelets or bone marrow megakaryocytes that contained growth-promoting factor .
	manualset3
90022	4	399000	13	NULL	NULL	0	NULL	peripheral platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there was no correlation between the colony-forming efficiency and the initial number of peripheral platelets or bone marrow megakaryocytes that contained growth-promoting factor .
	manualset3
90023	5	399000	13	NULL	NULL	0	NULL	bone marrow megakaryocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there was no correlation between the colony-forming efficiency and the initial number of peripheral platelets or bone marrow megakaryocytes that contained growth-promoting factor .
	manualset3
90024	6	399000	13	NULL	NULL	0	NULL	growth-promoting factor 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there was no correlation between the colony-forming efficiency and the initial number of peripheral platelets or bone marrow megakaryocytes that contained growth-promoting factor .
	manualset3
90025	1	399001	13	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there was no full correlation between ` retinoblastoma pathway ' inactivation and TA-p73 expression .
	manualset3
90026	2	399001	13	NULL	NULL	NULL	NULL	  ` retinoblastoma pathway ' inactivation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , there was no full correlation between ` retinoblastoma pathway ' inactivation and TA-p73 expression .
	manualset3
90027	3	399001	13	NULL	NULL	0	NULL	TA-p73 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , there was no full correlation between ` retinoblastoma pathway ' inactivation and TA-p73 expression .
	manualset3
90028	1	399002	13	NULL	NULL	0	NULL	oral administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , these changes were prevented by oral administration of PSK .
	manualset3
90029	2	399002	13	NULL	NULL	0	NULL	PSK	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , these changes were prevented by oral administration of PSK .
	manualset3
90030	1	399003	13	NULL	NULL	0	NULL	concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , these concentrations can inhibit the isolation of this microorganism but not its urease activity .
	manualset3
90031	2	399003	13	NULL	NULL	0	NULL	isolation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , these concentrations can inhibit the isolation of this microorganism but not its urease activity .
	manualset3
90032	3	399003	13	NULL	NULL	0	NULL	 microorganism	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , these concentrations can inhibit the isolation of this microorganism but not its urease activity .
	manualset3
90033	4	399003	13	NULL	NULL	0	NULL	urease activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , these concentrations can inhibit the isolation of this microorganism but not its urease activity .
	manualset3
90034	1	399004	13	NULL	NULL	0	NULL	factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , these different factors may elicit the same temporary or permanent response in that degenerating germ cells become more common , multinucleate giant germ cells form by coalescence of spermatocytes or spermatids , the ratio of germ cells to Sertoli cells is reduced , and spermatozoan production is adversely affected .
	manualset3
90035	2	399004	13	NULL	NULL	NULL	NULL	temporary or permanent response	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , these different factors may elicit the same temporary or permanent response in that degenerating germ cells become more common , multinucleate giant germ cells form by coalescence of spermatocytes or spermatids , the ratio of germ cells to Sertoli cells is reduced , and spermatozoan production is adversely affected .
	manualset3
90036	3	399004	13	NULL	NULL	NULL	NULL	degenerating germ cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , these different factors may elicit the same temporary or permanent response in that degenerating germ cells become more common , multinucleate giant germ cells form by coalescence of spermatocytes or spermatids , the ratio of germ cells to Sertoli cells is reduced , and spermatozoan production is adversely affected .
	manualset3
90037	4	399004	13	NULL	NULL	0	NULL	multinucleate giant germ cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , these different factors may elicit the same temporary or permanent response in that degenerating germ cells become more common , multinucleate giant germ cells form by coalescence of spermatocytes or spermatids , the ratio of germ cells to Sertoli cells is reduced , and spermatozoan production is adversely affected .
	manualset3
90038	5	399004	13	NULL	NULL	0	NULL	coalescence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , these different factors may elicit the same temporary or permanent response in that degenerating germ cells become more common , multinucleate giant germ cells form by coalescence of spermatocytes or spermatids , the ratio of germ cells to Sertoli cells is reduced , and spermatozoan production is adversely affected .
	manualset3
90039	6	399004	13	NULL	NULL	0	NULL	spermatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , these different factors may elicit the same temporary or permanent response in that degenerating germ cells become more common , multinucleate giant germ cells form by coalescence of spermatocytes or spermatids , the ratio of germ cells to Sertoli cells is reduced , and spermatozoan production is adversely affected .
	manualset3
90040	7	399004	13	NULL	NULL	0	NULL	 spermatids	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , these different factors may elicit the same temporary or permanent response in that degenerating germ cells become more common , multinucleate giant germ cells form by coalescence of spermatocytes or spermatids , the ratio of germ cells to Sertoli cells is reduced , and spermatozoan production is adversely affected .
	manualset3
90041	8	399004	13	NULL	NULL	0	NULL	ratio of germ cells to Sertoli cells 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , these different factors may elicit the same temporary or permanent response in that degenerating germ cells become more common , multinucleate giant germ cells form by coalescence of spermatocytes or spermatids , the ratio of germ cells to Sertoli cells is reduced , and spermatozoan production is adversely affected .
	manualset3
90042	9	399004	13	NULL	NULL	0	NULL	spermatozoan production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , these different factors may elicit the same temporary or permanent response in that degenerating germ cells become more common , multinucleate giant germ cells form by coalescence of spermatocytes or spermatids , the ratio of germ cells to Sertoli cells is reduced , and spermatozoan production is adversely affected .
	manualset3
90043	1	399005	13	NULL	NULL	NULL	NULL	ethnic-related differences 	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , these ethnic and gender-related differences were similar to those previously reported for ESRD in the general population .
	manualset3
90044	2	399005	13	NULL	NULL	0	NULL	ESRD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	However , these ethnic and gender-related differences were similar to those previously reported for ESRD in the general population .
	manualset3
90045	3	399005	13	NULL	NULL	NULL	NULL	 general population 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , these ethnic and gender-related differences were similar to those previously reported for ESRD in the general population .
	manualset3
90972	4	399005	13	NULL	NULL	0	NULL	gender-related differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	However , these ethnic and gender-related differences were similar to those previously reported for ESRD in the general population .
	manualset3
90046	1	399006	13	NULL	NULL	0	NULL	modalities 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , these modalities only provide anatomical information of the coronary artery .
	manualset3
90047	2	399006	13	NULL	NULL	NULL	NULL	anatomical information	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , these modalities only provide anatomical information of the coronary artery .
	manualset3
90048	3	399006	13	NULL	NULL	0	NULL	 coronary artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , these modalities only provide anatomical information of the coronary artery .
	manualset3
90049	1	399007	13	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , these studies were conducted in university teaching hospitals whereas a significant proportion of training in Ireland takes place in peripheral hospitals which provide a different training environment .
	manualset3
90050	2	399007	13	NULL	NULL	0	NULL	university teaching hospitals	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	However , these studies were conducted in university teaching hospitals whereas a significant proportion of training in Ireland takes place in peripheral hospitals which provide a different training environment .
	manualset3
90051	3	399007	13	NULL	NULL	0	NULL	proportion	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , these studies were conducted in university teaching hospitals whereas a significant proportion of training in Ireland takes place in peripheral hospitals which provide a different training environment .
	manualset3
90052	4	399007	13	NULL	NULL	0	NULL	training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , these studies were conducted in university teaching hospitals whereas a significant proportion of training in Ireland takes place in peripheral hospitals which provide a different training environment .
	manualset3
90053	5	399007	13	NULL	NULL	0	NULL	Ireland	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , these studies were conducted in university teaching hospitals whereas a significant proportion of training in Ireland takes place in peripheral hospitals which provide a different training environment .
	manualset3
90054	6	399007	13	NULL	NULL	NULL	NULL	 peripheral hospitals	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , these studies were conducted in university teaching hospitals whereas a significant proportion of training in Ireland takes place in peripheral hospitals which provide a different training environment .
	manualset3
90055	7	399007	13	NULL	NULL	0	NULL	training environment 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , these studies were conducted in university teaching hospitals whereas a significant proportion of training in Ireland takes place in peripheral hospitals which provide a different training environment .
	manualset3
90056	1	399008	13	NULL	NULL	0	NULL	 information 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	However , they can give information of a more general nature - much in the same way as measurements of tension may do , for example - and the patterns can also tell us what structural regularities are no longer present during contraction .
	manualset3
90057	2	399008	13	NULL	NULL	NULL	NULL	measurements of tension	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , they can give information of a more general nature - much in the same way as measurements of tension may do , for example - and the patterns can also tell us what structural regularities are no longer present during contraction .
	manualset3
90058	3	399008	13	NULL	NULL	0	NULL	 patterns	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , they can give information of a more general nature - much in the same way as measurements of tension may do , for example - and the patterns can also tell us what structural regularities are no longer present during contraction .
	manualset3
90059	4	399008	13	NULL	NULL	NULL	NULL	general nature	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , they can give information of a more general nature - much in the same way as measurements of tension may do , for example - and the patterns can also tell us what structural regularities are no longer present during contraction .
	manualset3
90060	5	399008	13	NULL	NULL	0	NULL	contraction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , they can give information of a more general nature - much in the same way as measurements of tension may do , for example - and the patterns can also tell us what structural regularities are no longer present during contraction .
	manualset3
91217	6	399008	13	NULL	NULL	0	NULL	structural regularities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , they can give information of a more general nature - much in the same way as measurements of tension may do , for example - and the patterns can also tell us what structural regularities are no longer present during contraction .
	manualset3
90061	1	399009	13	NULL	NULL	NULL	NULL	allogeneic transplantation 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , they have been clinically beneficial in allogeneic transplantation and in delayed erythropoiesis post-transplantation .
	manualset3
90062	2	399009	13	NULL	NULL	0	NULL	erythropoiesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , they have been clinically beneficial in allogeneic transplantation and in delayed erythropoiesis post-transplantation .
	manualset3
90063	3	399009	13	NULL	NULL	0	NULL	post-transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , they have been clinically beneficial in allogeneic transplantation and in delayed erythropoiesis post-transplantation .
	manualset3
90064	1	399010	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , they have not been employed in the treatment of central hyperthyroidism .
	manualset3
90065	2	399010	13	NULL	NULL	NULL	NULL	central hyperthyroidism	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , they have not been employed in the treatment of central hyperthyroidism .
	manualset3
90066	1	399011	13	NULL	NULL	0	NULL	 risk factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , they suggest for the first time that individual risk factors related to the HPA axis predict stereotypic behavior following enrichment-removal , and that previously-enriched mice have lasting motivational differences from standard-raised mice , suggesting sustained behavioural effects related to the frustration of enrichment-loss .
	manualset3
90067	2	399011	13	NULL	NULL	0	NULL	HPA axis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , they suggest for the first time that individual risk factors related to the HPA axis predict stereotypic behavior following enrichment-removal , and that previously-enriched mice have lasting motivational differences from standard-raised mice , suggesting sustained behavioural effects related to the frustration of enrichment-loss .
	manualset3
90068	3	399011	13	NULL	NULL	NULL	NULL	stereotypic behavior	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , they suggest for the first time that individual risk factors related to the HPA axis predict stereotypic behavior following enrichment-removal , and that previously-enriched mice have lasting motivational differences from standard-raised mice , suggesting sustained behavioural effects related to the frustration of enrichment-loss .
	manualset3
90069	4	399011	13	NULL	NULL	0	NULL	enrichment-removal 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , they suggest for the first time that individual risk factors related to the HPA axis predict stereotypic behavior following enrichment-removal , and that previously-enriched mice have lasting motivational differences from standard-raised mice , suggesting sustained behavioural effects related to the frustration of enrichment-loss .
	manualset3
90070	5	399011	13	NULL	NULL	0	NULL	 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , they suggest for the first time that individual risk factors related to the HPA axis predict stereotypic behavior following enrichment-removal , and that previously-enriched mice have lasting motivational differences from standard-raised mice , suggesting sustained behavioural effects related to the frustration of enrichment-loss .
	manualset3
90071	6	399011	13	NULL	NULL	NULL	NULL	motivational differences	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , they suggest for the first time that individual risk factors related to the HPA axis predict stereotypic behavior following enrichment-removal , and that previously-enriched mice have lasting motivational differences from standard-raised mice , suggesting sustained behavioural effects related to the frustration of enrichment-loss .
	manualset3
90072	7	399011	13	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , they suggest for the first time that individual risk factors related to the HPA axis predict stereotypic behavior following enrichment-removal , and that previously-enriched mice have lasting motivational differences from standard-raised mice , suggesting sustained behavioural effects related to the frustration of enrichment-loss .
	manualset3
90073	8	399011	13	NULL	NULL	0	NULL	behavioural effects 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , they suggest for the first time that individual risk factors related to the HPA axis predict stereotypic behavior following enrichment-removal , and that previously-enriched mice have lasting motivational differences from standard-raised mice , suggesting sustained behavioural effects related to the frustration of enrichment-loss .
	manualset3
90074	9	399011	13	NULL	NULL	NULL	NULL	frustration of enrichment-loss	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , they suggest for the first time that individual risk factors related to the HPA axis predict stereotypic behavior following enrichment-removal , and that previously-enriched mice have lasting motivational differences from standard-raised mice , suggesting sustained behavioural effects related to the frustration of enrichment-loss .
	manualset3
90076	1	399012	13	NULL	NULL	0	NULL	case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , this case differs in that the patient had no preexisting gynecologic conditions at the time of hysterectomy and bilateral salpingo-oophorectomy to account for residual ovarian tissue .
	manualset3
90077	2	399012	13	NULL	NULL	0	NULL	patient	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , this case differs in that the patient had no preexisting gynecologic conditions at the time of hysterectomy and bilateral salpingo-oophorectomy to account for residual ovarian tissue .
	manualset3
90078	3	399012	13	NULL	NULL	NULL	NULL	gynecologic conditions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , this case differs in that the patient had no preexisting gynecologic conditions at the time of hysterectomy and bilateral salpingo-oophorectomy to account for residual ovarian tissue .
	manualset3
90079	4	399012	13	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	However , this case differs in that the patient had no preexisting gynecologic conditions at the time of hysterectomy and bilateral salpingo-oophorectomy to account for residual ovarian tissue .
	manualset3
90080	5	399012	13	NULL	NULL	0	NULL	hysterectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , this case differs in that the patient had no preexisting gynecologic conditions at the time of hysterectomy and bilateral salpingo-oophorectomy to account for residual ovarian tissue .
	manualset3
90081	6	399012	13	NULL	NULL	NULL	NULL	bilateral salpingo-oophorectomy 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , this case differs in that the patient had no preexisting gynecologic conditions at the time of hysterectomy and bilateral salpingo-oophorectomy to account for residual ovarian tissue .
	manualset3
90082	7	399012	13	NULL	NULL	NULL	NULL	 residual ovarian tissue	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , this case differs in that the patient had no preexisting gynecologic conditions at the time of hysterectomy and bilateral salpingo-oophorectomy to account for residual ovarian tissue .
	manualset3
90083	1	399013	13	NULL	NULL	0	NULL	fragment	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	However , this fragment did not contain the oprD structural gene as judged by its inability to hybridize with an oligonucleotide corresponding to the N-terminal amino acid sequence of OprD .
	manualset3
90084	2	399013	13	NULL	NULL	0	NULL	oprD structural gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	However , this fragment did not contain the oprD structural gene as judged by its inability to hybridize with an oligonucleotide corresponding to the N-terminal amino acid sequence of OprD .
	manualset3
90086	4	399013	13	NULL	NULL	0	NULL	oligonucleotide	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	However , this fragment did not contain the oprD structural gene as judged by its inability to hybridize with an oligonucleotide corresponding to the N-terminal amino acid sequence of OprD .
	manualset3
90087	5	399013	13	NULL	NULL	0	NULL	N-terminal amino acid sequence of OprD	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	However , this fragment did not contain the oprD structural gene as judged by its inability to hybridize with an oligonucleotide corresponding to the N-terminal amino acid sequence of OprD .
	manualset3
90088	1	399014	13	NULL	NULL	NULL	NULL	prior history of depression	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , those with prior history of depression may face a re-emergence of depression during this transition while others may experience a first episode of depression in their lives .
	manualset3
90090	3	399014	13	NULL	NULL	NULL	NULL	 re-emergence of depression 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , those with prior history of depression may face a re-emergence of depression during this transition while others may experience a first episode of depression in their lives .
	manualset3
90092	5	399014	13	NULL	NULL	0	NULL	transition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , those with prior history of depression may face a re-emergence of depression during this transition while others may experience a first episode of depression in their lives .
	manualset3
90093	6	399014	13	NULL	NULL	0	NULL	experience	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , those with prior history of depression may face a re-emergence of depression during this transition while others may experience a first episode of depression in their lives .
	manualset3
90094	7	399014	13	NULL	NULL	0	NULL	first episode of depression 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , those with prior history of depression may face a re-emergence of depression during this transition while others may experience a first episode of depression in their lives .
	manualset3
90095	8	399014	13	NULL	NULL	0	NULL	lives	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , those with prior history of depression may face a re-emergence of depression during this transition while others may experience a first episode of depression in their lives .
	manualset3
90096	1	399015	13	NULL	NULL	0	NULL	attention 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , though much attention has been given to infrapopliteal intervention , the importance of identifying preprocedural infrapopliteal variants remains underappreciated .
	manualset3
90097	2	399015	13	NULL	NULL	0	NULL	 infrapopliteal intervention 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , though much attention has been given to infrapopliteal intervention , the importance of identifying preprocedural infrapopliteal variants remains underappreciated .
	manualset3
90098	3	399015	13	NULL	NULL	NULL	NULL	preprocedural infrapopliteal variants	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , though much attention has been given to infrapopliteal intervention , the importance of identifying preprocedural infrapopliteal variants remains underappreciated .
	manualset3
90099	1	399016	13	NULL	NULL	0	NULL	three of the four individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , three of the four individuals developed extensive areas of acanthosis nigricans beginning in early childhood , suffer from severe neurological impairments , and have survived past infancy without prolonged life-support measures .
	manualset3
90100	2	399016	13	NULL	NULL	0	NULL	areas of acanthosis nigricans	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , three of the four individuals developed extensive areas of acanthosis nigricans beginning in early childhood , suffer from severe neurological impairments , and have survived past infancy without prolonged life-support measures .
	manualset3
90101	3	399016	13	NULL	NULL	NULL	NULL	early childhood	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , three of the four individuals developed extensive areas of acanthosis nigricans beginning in early childhood , suffer from severe neurological impairments , and have survived past infancy without prolonged life-support measures .
	manualset3
90102	4	399016	13	NULL	NULL	0	NULL	neurological impairments 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , three of the four individuals developed extensive areas of acanthosis nigricans beginning in early childhood , suffer from severe neurological impairments , and have survived past infancy without prolonged life-support measures .
	manualset3
90103	5	399016	13	NULL	NULL	0	NULL	 infancy 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	However , three of the four individuals developed extensive areas of acanthosis nigricans beginning in early childhood , suffer from severe neurological impairments , and have survived past infancy without prolonged life-support measures .
	manualset3
90104	6	399016	13	NULL	NULL	0	NULL	life-support measures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , three of the four individuals developed extensive areas of acanthosis nigricans beginning in early childhood , suffer from severe neurological impairments , and have survived past infancy without prolonged life-support measures .
	manualset3
90105	1	399017	13	NULL	NULL	0	NULL	date 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	However , to date only a limited number of P450s have been identified and characterized in legumes .
	manualset3
90106	2	399017	13	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , to date only a limited number of P450s have been identified and characterized in legumes .
	manualset3
90107	3	399017	13	NULL	NULL	0	NULL	P450s 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , to date only a limited number of P450s have been identified and characterized in legumes .
	manualset3
90108	4	399017	13	NULL	NULL	0	NULL	legumes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , to date only a limited number of P450s have been identified and characterized in legumes .
	manualset3
90109	1	399018	13	NULL	NULL	0	NULL	molecular details 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , to understand the molecular details of microglia activation , future work is required .
	manualset3
90110	2	399018	13	NULL	NULL	NULL	NULL	microglia activation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , to understand the molecular details of microglia activation , future work is required .
	manualset3
90111	3	399018	13	NULL	NULL	0	NULL	future work	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , to understand the molecular details of microglia activation , future work is required .
	manualset3
90112	1	399019	13	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , two misdiagnoses have been also described , showing the need for further development and improvement in the accuracy , efficiency and efficacy of DNA analysis in single cells .
	manualset3
90113	2	399019	13	NULL	NULL	0	NULL	development in the accuracy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , two misdiagnoses have been also described , showing the need for further development and improvement in the accuracy , efficiency and efficacy of DNA analysis in single cells .
	manualset3
90114	3	399019	13	NULL	NULL	0	NULL	improvement in the accuracy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , two misdiagnoses have been also described , showing the need for further development and improvement in the accuracy , efficiency and efficacy of DNA analysis in single cells .
	manualset3
90115	4	399019	13	NULL	NULL	0	NULL	efficiency of DNA analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , two misdiagnoses have been also described , showing the need for further development and improvement in the accuracy , efficiency and efficacy of DNA analysis in single cells .
	manualset3
90116	5	399019	13	NULL	NULL	0	NULL	efficacy of DNA analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , two misdiagnoses have been also described , showing the need for further development and improvement in the accuracy , efficiency and efficacy of DNA analysis in single cells .
	manualset3
90117	6	399019	13	NULL	NULL	NULL	NULL	single cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , two misdiagnoses have been also described , showing the need for further development and improvement in the accuracy , efficiency and efficacy of DNA analysis in single cells .
	manualset3
91240	7	399019	13	NULL	NULL	0	NULL	 misdiagnoses 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , two misdiagnoses have been also described , showing the need for further development and improvement in the accuracy , efficiency and efficacy of DNA analysis in single cells .
	manualset3
90118	1	399020	13	NULL	NULL	0	NULL	nurse	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( The nurse and the community ) .
	manualset3
90119	2	399020	13	NULL	NULL	0	NULL	community	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( The nurse and the community ) .
	manualset3
90120	1	399021	13	NULL	NULL	0	NULL	exons 1-CAT hybrid mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	However , unexpectedly exons 1-CAT hybrid mRNA in JEG-3 cells was not induced by forskolin .
	manualset3
90121	2	399021	13	NULL	NULL	0	NULL	JEG-3 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , unexpectedly exons 1-CAT hybrid mRNA in JEG-3 cells was not induced by forskolin .
	manualset3
90122	3	399021	13	NULL	NULL	0	NULL	forskolin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , unexpectedly exons 1-CAT hybrid mRNA in JEG-3 cells was not induced by forskolin .
	manualset3
90123	1	399022	13	NULL	NULL	0	NULL	C7H9 + 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	However , unlike for C7H9 + both the bishomo square pyramidal structure 3 and the trishomocyclopropenium type structure 4 were found to be minima on the potential energy surface of C8H9 + .
	manualset3
90124	2	399022	13	NULL	NULL	0	NULL	bishomo square pyramidal structure 3 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	However , unlike for C7H9 + both the bishomo square pyramidal structure 3 and the trishomocyclopropenium type structure 4 were found to be minima on the potential energy surface of C8H9 + .
	manualset3
90125	3	399022	13	NULL	NULL	0	NULL	trishomocyclopropenium type structure 4 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	However , unlike for C7H9 + both the bishomo square pyramidal structure 3 and the trishomocyclopropenium type structure 4 were found to be minima on the potential energy surface of C8H9 + .
	manualset3
90126	4	399022	13	NULL	NULL	0	NULL	minima	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , unlike for C7H9 + both the bishomo square pyramidal structure 3 and the trishomocyclopropenium type structure 4 were found to be minima on the potential energy surface of C8H9 + .
	manualset3
90127	5	399022	13	NULL	NULL	NULL	NULL	potential energy surface	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , unlike for C7H9 + both the bishomo square pyramidal structure 3 and the trishomocyclopropenium type structure 4 were found to be minima on the potential energy surface of C8H9 + .
	manualset3
90128	6	399022	13	NULL	NULL	0	NULL	C8H9 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	However , unlike for C7H9 + both the bishomo square pyramidal structure 3 and the trishomocyclopropenium type structure 4 were found to be minima on the potential energy surface of C8H9 + .
	manualset3
90129	1	399023	13	NULL	NULL	0	NULL	cGMP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , we demonstrate that cGMP can directly activate PDE5 without phosphorylation in platelet cytosol , most likely via binding to the regulatory GAF domains .
	manualset3
90130	2	399023	13	NULL	NULL	0	NULL	PDE5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , we demonstrate that cGMP can directly activate PDE5 without phosphorylation in platelet cytosol , most likely via binding to the regulatory GAF domains .
	manualset3
90131	3	399023	13	NULL	NULL	0	NULL	phosphorylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , we demonstrate that cGMP can directly activate PDE5 without phosphorylation in platelet cytosol , most likely via binding to the regulatory GAF domains .
	manualset3
90132	4	399023	13	NULL	NULL	0	NULL	platelet cytosol	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	However , we demonstrate that cGMP can directly activate PDE5 without phosphorylation in platelet cytosol , most likely via binding to the regulatory GAF domains .
	manualset3
90133	5	399023	13	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , we demonstrate that cGMP can directly activate PDE5 without phosphorylation in platelet cytosol , most likely via binding to the regulatory GAF domains .
	manualset3
90134	6	399023	13	NULL	NULL	0	NULL	regulatory GAF domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , we demonstrate that cGMP can directly activate PDE5 without phosphorylation in platelet cytosol , most likely via binding to the regulatory GAF domains .
	manualset3
90135	1	399024	13	NULL	NULL	0	NULL	DYS287 YAP + individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , we did find DYS287 YAP + individuals who harbored the DYS199 C allele in one Native American population , the Mixe , and in one Asian group , the Tibetans .
	manualset3
90136	2	399024	13	NULL	NULL	NULL	NULL	 DYS199 C allele	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , we did find DYS287 YAP + individuals who harbored the DYS199 C allele in one Native American population , the Mixe , and in one Asian group , the Tibetans .
	manualset3
90137	3	399024	13	NULL	NULL	NULL	NULL	one Native American population	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , we did find DYS287 YAP + individuals who harbored the DYS199 C allele in one Native American population , the Mixe , and in one Asian group , the Tibetans .
	manualset3
90138	4	399024	13	NULL	NULL	0	NULL	Mixe	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , we did find DYS287 YAP + individuals who harbored the DYS199 C allele in one Native American population , the Mixe , and in one Asian group , the Tibetans .
	manualset3
90139	5	399024	13	NULL	NULL	0	NULL	one Asian group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , we did find DYS287 YAP + individuals who harbored the DYS199 C allele in one Native American population , the Mixe , and in one Asian group , the Tibetans .
	manualset3
90140	6	399024	13	NULL	NULL	0	NULL	Tibetans	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , we did find DYS287 YAP + individuals who harbored the DYS199 C allele in one Native American population , the Mixe , and in one Asian group , the Tibetans .
	manualset3
90141	1	399025	13	NULL	NULL	0	NULL	mouse chow	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	However , we discovered that most normal mouse chow contains casein .
	manualset3
90142	2	399025	13	NULL	NULL	0	NULL	casein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , we discovered that most normal mouse chow contains casein .
	manualset3
90143	1	399026	13	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , we failed to detect evidence of strong positive selection in any of the cas genes .
	manualset3
90144	2	399026	13	NULL	NULL	0	NULL	selection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , we failed to detect evidence of strong positive selection in any of the cas genes .
	manualset3
90145	3	399026	13	NULL	NULL	0	NULL	cas genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , we failed to detect evidence of strong positive selection in any of the cas genes .
	manualset3
90146	1	399027	13	NULL	NULL	0	NULL	steroid hormone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , we now know that this steroid hormone activates multiple signaling pathways to affect neuronal excitability and gene transcription .
	manualset3
90147	2	399027	13	NULL	NULL	NULL	NULL	multiple signaling pathways 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , we now know that this steroid hormone activates multiple signaling pathways to affect neuronal excitability and gene transcription .
	manualset3
90148	3	399027	13	NULL	NULL	0	NULL	neuronal excitability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , we now know that this steroid hormone activates multiple signaling pathways to affect neuronal excitability and gene transcription .
	manualset3
90149	4	399027	13	NULL	NULL	0	NULL	gene transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , we now know that this steroid hormone activates multiple signaling pathways to affect neuronal excitability and gene transcription .
	manualset3
90150	1	399028	13	NULL	NULL	0	NULL	 surface scatter	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	However , we show that surface scatter can be treated very similarly to conventional wavefront aberrations .
	manualset3
90151	2	399028	13	NULL	NULL	0	NULL	wavefront aberrations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , we show that surface scatter can be treated very similarly to conventional wavefront aberrations .
	manualset3
90152	1	399029	13	NULL	NULL	0	NULL	cell-associated gp41 molecules 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , we suggest that only a minority of cell-associated gp41 molecules - those destined for incorporation into virions - has 3 MSDs and the minor ectodomain .
	manualset3
90153	2	399029	13	NULL	NULL	0	NULL	incorporation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , we suggest that only a minority of cell-associated gp41 molecules - those destined for incorporation into virions - has 3 MSDs and the minor ectodomain .
	manualset3
90154	3	399029	13	NULL	NULL	0	NULL	virions 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , we suggest that only a minority of cell-associated gp41 molecules - those destined for incorporation into virions - has 3 MSDs and the minor ectodomain .
	manualset3
90155	4	399029	13	NULL	NULL	0	NULL	3 MSDs	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , we suggest that only a minority of cell-associated gp41 molecules - those destined for incorporation into virions - has 3 MSDs and the minor ectodomain .
	manualset3
90156	5	399029	13	NULL	NULL	NULL	NULL	minor ectodomain	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , we suggest that only a minority of cell-associated gp41 molecules - those destined for incorporation into virions - has 3 MSDs and the minor ectodomain .
	manualset3
90157	1	399030	13	NULL	NULL	0	NULL	protein crystals	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , we were able to obtain protein crystals suited for X-ray structure determination from flavodoxin expressed as an intein-CBD fusion protein , but not from flavodoxin expressed with a C-terminal His ( 6 ) - tag .
	manualset3
90158	2	399030	13	NULL	NULL	0	NULL	X-ray structure determination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , we were able to obtain protein crystals suited for X-ray structure determination from flavodoxin expressed as an intein-CBD fusion protein , but not from flavodoxin expressed with a C-terminal His ( 6 ) - tag .
	manualset3
90159	3	399030	13	NULL	NULL	0	NULL	flavodoxin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , we were able to obtain protein crystals suited for X-ray structure determination from flavodoxin expressed as an intein-CBD fusion protein , but not from flavodoxin expressed with a C-terminal His ( 6 ) - tag .
	manualset3
90160	4	399030	13	NULL	NULL	0	NULL	intein-CBD fusion protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , we were able to obtain protein crystals suited for X-ray structure determination from flavodoxin expressed as an intein-CBD fusion protein , but not from flavodoxin expressed with a C-terminal His ( 6 ) - tag .
	manualset3
90161	5	399030	13	NULL	NULL	NULL	NULL	flavodoxin expressed with a C-terminal His ( 6 ) - tag	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , we were able to obtain protein crystals suited for X-ray structure determination from flavodoxin expressed as an intein-CBD fusion protein , but not from flavodoxin expressed with a C-terminal His ( 6 ) - tag .
	manualset3
90188	1	399031	13	NULL	NULL	0	NULL	ventilator settings	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , what is true for ventilator settings should also be true for extracorporeal procedures : studies will have to demonstrate a convincing risk-benefit ratio .
	manualset3
90189	2	399031	13	NULL	NULL	NULL	NULL	extracorporeal procedures	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , what is true for ventilator settings should also be true for extracorporeal procedures : studies will have to demonstrate a convincing risk-benefit ratio .
	manualset3
90190	3	399031	13	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , what is true for ventilator settings should also be true for extracorporeal procedures : studies will have to demonstrate a convincing risk-benefit ratio .
	manualset3
90191	4	399031	13	NULL	NULL	0	NULL	risk-benefit ratio	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , what is true for ventilator settings should also be true for extracorporeal procedures : studies will have to demonstrate a convincing risk-benefit ratio .
	manualset3
90192	1	399032	13	NULL	NULL	0	NULL	level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when divided according to potential level of IL-10 production , the group of potentially high IL-10 producers among the CD patients demonstrated significantly lower levels of antitissue transglutaminase antibodies compared to potentially low IL-10 producers ( p = 0.01 ) .
	manualset3
90193	2	399032	13	NULL	NULL	0	NULL	 IL-10 production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when divided according to potential level of IL-10 production , the group of potentially high IL-10 producers among the CD patients demonstrated significantly lower levels of antitissue transglutaminase antibodies compared to potentially low IL-10 producers ( p = 0.01 ) .
	manualset3
90194	3	399032	13	NULL	NULL	NULL	NULL	group 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , when divided according to potential level of IL-10 production , the group of potentially high IL-10 producers among the CD patients demonstrated significantly lower levels of antitissue transglutaminase antibodies compared to potentially low IL-10 producers ( p = 0.01 ) .
	manualset3
90195	4	399032	13	NULL	NULL	0	NULL	IL-10 producers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when divided according to potential level of IL-10 production , the group of potentially high IL-10 producers among the CD patients demonstrated significantly lower levels of antitissue transglutaminase antibodies compared to potentially low IL-10 producers ( p = 0.01 ) .
	manualset3
90196	5	399032	13	NULL	NULL	0	NULL	CD patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when divided according to potential level of IL-10 production , the group of potentially high IL-10 producers among the CD patients demonstrated significantly lower levels of antitissue transglutaminase antibodies compared to potentially low IL-10 producers ( p = 0.01 ) .
	manualset3
90197	6	399032	13	NULL	NULL	0	NULL	 levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when divided according to potential level of IL-10 production , the group of potentially high IL-10 producers among the CD patients demonstrated significantly lower levels of antitissue transglutaminase antibodies compared to potentially low IL-10 producers ( p = 0.01 ) .
	manualset3
90198	7	399032	13	NULL	NULL	NULL	NULL	antitissue transglutaminase antibodies	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , when divided according to potential level of IL-10 production , the group of potentially high IL-10 producers among the CD patients demonstrated significantly lower levels of antitissue transglutaminase antibodies compared to potentially low IL-10 producers ( p = 0.01 ) .
	manualset3
90199	8	399032	13	NULL	NULL	0	NULL	IL-10 producers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when divided according to potential level of IL-10 production , the group of potentially high IL-10 producers among the CD patients demonstrated significantly lower levels of antitissue transglutaminase antibodies compared to potentially low IL-10 producers ( p = 0.01 ) .
	manualset3
90200	9	399032	13	NULL	NULL	0	NULL	p = 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when divided according to potential level of IL-10 production , the group of potentially high IL-10 producers among the CD patients demonstrated significantly lower levels of antitissue transglutaminase antibodies compared to potentially low IL-10 producers ( p = 0.01 ) .
	manualset3
90201	1	399033	13	NULL	NULL	0	NULL	histamine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when histamine was present in combination with isoproterenol or forskolin 4-DAMP mustard treatment shifted the concentration-effect curves for oxo-M to the right only about 3.5-fold .
	manualset3
90202	2	399033	13	NULL	NULL	NULL	NULL	isoproterenol 	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , when histamine was present in combination with isoproterenol or forskolin 4-DAMP mustard treatment shifted the concentration-effect curves for oxo-M to the right only about 3.5-fold .
	manualset3
90203	3	399033	13	NULL	NULL	NULL	NULL	 forskolin	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , when histamine was present in combination with isoproterenol or forskolin 4-DAMP mustard treatment shifted the concentration-effect curves for oxo-M to the right only about 3.5-fold .
	manualset3
90204	4	399033	13	NULL	NULL	NULL	NULL	4-DAMP mustard	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , when histamine was present in combination with isoproterenol or forskolin 4-DAMP mustard treatment shifted the concentration-effect curves for oxo-M to the right only about 3.5-fold .
	manualset3
90205	5	399033	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when histamine was present in combination with isoproterenol or forskolin 4-DAMP mustard treatment shifted the concentration-effect curves for oxo-M to the right only about 3.5-fold .
	manualset3
90206	6	399033	13	NULL	NULL	NULL	NULL	concentration-effect curves	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , when histamine was present in combination with isoproterenol or forskolin 4-DAMP mustard treatment shifted the concentration-effect curves for oxo-M to the right only about 3.5-fold .
	manualset3
90207	7	399033	13	NULL	NULL	0	NULL	 oxo-M 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when histamine was present in combination with isoproterenol or forskolin 4-DAMP mustard treatment shifted the concentration-effect curves for oxo-M to the right only about 3.5-fold .
	manualset3
90208	8	399033	13	NULL	NULL	0	NULL	3.5-fold 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when histamine was present in combination with isoproterenol or forskolin 4-DAMP mustard treatment shifted the concentration-effect curves for oxo-M to the right only about 3.5-fold .
	manualset3
90209	1	399034	13	NULL	NULL	0	NULL	lysis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when lysis was induced by the isolated C5b-9 membrane attack mechanism , bypassing the requirement for C3 binding , only type III PNH cells exhibited greater than normal lysis .
	manualset3
90210	2	399034	13	NULL	NULL	NULL	NULL	C5b-9 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , when lysis was induced by the isolated C5b-9 membrane attack mechanism , bypassing the requirement for C3 binding , only type III PNH cells exhibited greater than normal lysis .
	manualset3
90211	3	399034	13	NULL	NULL	NULL	NULL	membrane attack mechanism	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , when lysis was induced by the isolated C5b-9 membrane attack mechanism , bypassing the requirement for C3 binding , only type III PNH cells exhibited greater than normal lysis .
	manualset3
90226	5	399034	13	NULL	NULL	0	NULL	C3 binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when lysis was induced by the isolated C5b-9 membrane attack mechanism , bypassing the requirement for C3 binding , only type III PNH cells exhibited greater than normal lysis .
	manualset3
90227	6	399034	13	NULL	NULL	0	NULL	type III PNH cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when lysis was induced by the isolated C5b-9 membrane attack mechanism , bypassing the requirement for C3 binding , only type III PNH cells exhibited greater than normal lysis .
	manualset3
90228	7	399034	13	NULL	NULL	0	NULL	lysis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when lysis was induced by the isolated C5b-9 membrane attack mechanism , bypassing the requirement for C3 binding , only type III PNH cells exhibited greater than normal lysis .
	manualset3
90229	1	399035	13	NULL	NULL	0	NULL	peripheral blood mononuclear cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when peripheral blood mononuclear cells and B lymphocytes are isolated from BLV-infected animals and incubated in the presence of activating reagents , such as phorbol ester , the expression of BLV is markedly enhanced .
	manualset3
90230	2	399035	13	NULL	NULL	0	NULL	B lymphocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when peripheral blood mononuclear cells and B lymphocytes are isolated from BLV-infected animals and incubated in the presence of activating reagents , such as phorbol ester , the expression of BLV is markedly enhanced .
	manualset3
90231	3	399035	13	NULL	NULL	0	NULL	BLV-infected animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when peripheral blood mononuclear cells and B lymphocytes are isolated from BLV-infected animals and incubated in the presence of activating reagents , such as phorbol ester , the expression of BLV is markedly enhanced .
	manualset3
90232	4	399035	13	NULL	NULL	NULL	NULL	activating reagents	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , when peripheral blood mononuclear cells and B lymphocytes are isolated from BLV-infected animals and incubated in the presence of activating reagents , such as phorbol ester , the expression of BLV is markedly enhanced .
	manualset3
90233	5	399035	13	NULL	NULL	0	NULL	 phorbol ester	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when peripheral blood mononuclear cells and B lymphocytes are isolated from BLV-infected animals and incubated in the presence of activating reagents , such as phorbol ester , the expression of BLV is markedly enhanced .
	manualset3
90234	6	399035	13	NULL	NULL	0	NULL	expression of BLV 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when peripheral blood mononuclear cells and B lymphocytes are isolated from BLV-infected animals and incubated in the presence of activating reagents , such as phorbol ester , the expression of BLV is markedly enhanced .
	manualset3
90235	1	399036	13	NULL	NULL	0	NULL	pathogenesis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( The pathogenesis of CD4 ( + ) ; T cells infiltrated into the spinal cord in rat SNL model ) .
	manualset3
90236	2	399036	13	NULL	NULL	NULL	NULL	CD4 ( + ) ; T cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The pathogenesis of CD4 ( + ) ; T cells infiltrated into the spinal cord in rat SNL model ) .
	manualset3
90238	4	399036	13	NULL	NULL	0	NULL	spinal cord	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( The pathogenesis of CD4 ( + ) ; T cells infiltrated into the spinal cord in rat SNL model ) .
	manualset3
90239	5	399036	13	NULL	NULL	0	NULL	rat SNL model 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( The pathogenesis of CD4 ( + ) ; T cells infiltrated into the spinal cord in rat SNL model ) .
	manualset3
90240	1	399037	13	NULL	NULL	0	NULL	 mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when tested in mice bearing tumor cells expressing mesothelin , the antitumor activity of the bivalent immunotoxin is very similar to the activity of the lower affinity monovalent immunotoxin .
	manualset3
90241	2	399037	13	NULL	NULL	0	NULL	tumor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when tested in mice bearing tumor cells expressing mesothelin , the antitumor activity of the bivalent immunotoxin is very similar to the activity of the lower affinity monovalent immunotoxin .
	manualset3
90242	3	399037	13	NULL	NULL	0	NULL	 mesothelin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when tested in mice bearing tumor cells expressing mesothelin , the antitumor activity of the bivalent immunotoxin is very similar to the activity of the lower affinity monovalent immunotoxin .
	manualset3
90244	4	399037	13	NULL	NULL	0	NULL	antitumor activity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when tested in mice bearing tumor cells expressing mesothelin , the antitumor activity of the bivalent immunotoxin is very similar to the activity of the lower affinity monovalent immunotoxin .
	manualset3
90246	5	399037	13	NULL	NULL	NULL	NULL	bivalent immunotoxin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , when tested in mice bearing tumor cells expressing mesothelin , the antitumor activity of the bivalent immunotoxin is very similar to the activity of the lower affinity monovalent immunotoxin .
	manualset3
90249	6	399037	13	NULL	NULL	NULL	NULL	activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , when tested in mice bearing tumor cells expressing mesothelin , the antitumor activity of the bivalent immunotoxin is very similar to the activity of the lower affinity monovalent immunotoxin .
	manualset3
90250	7	399037	13	NULL	NULL	0	NULL	affinity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when tested in mice bearing tumor cells expressing mesothelin , the antitumor activity of the bivalent immunotoxin is very similar to the activity of the lower affinity monovalent immunotoxin .
	manualset3
90251	8	399037	13	NULL	NULL	NULL	NULL	monovalent immunotoxin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , when tested in mice bearing tumor cells expressing mesothelin , the antitumor activity of the bivalent immunotoxin is very similar to the activity of the lower affinity monovalent immunotoxin .
	manualset3
90266	1	399038	13	NULL	NULL	0	NULL	electrode	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when the electrode was placed on the nasal ala , the threshold was significantly lower , an ideal biphasic configuration was present in almost all cases ( 97.5 per cent ) of normal volunteers and it was easier to identify the waveform .
	manualset3
90268	2	399038	13	NULL	NULL	0	NULL	nasal ala	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when the electrode was placed on the nasal ala , the threshold was significantly lower , an ideal biphasic configuration was present in almost all cases ( 97.5 per cent ) of normal volunteers and it was easier to identify the waveform .
	manualset3
90270	3	399038	13	NULL	NULL	0	NULL	 threshold 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when the electrode was placed on the nasal ala , the threshold was significantly lower , an ideal biphasic configuration was present in almost all cases ( 97.5 per cent ) of normal volunteers and it was easier to identify the waveform .
	manualset3
90272	4	399038	13	NULL	NULL	NULL	NULL	biphasic configuration 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , when the electrode was placed on the nasal ala , the threshold was significantly lower , an ideal biphasic configuration was present in almost all cases ( 97.5 per cent ) of normal volunteers and it was easier to identify the waveform .
	manualset3
90273	5	399038	13	NULL	NULL	0	NULL	 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when the electrode was placed on the nasal ala , the threshold was significantly lower , an ideal biphasic configuration was present in almost all cases ( 97.5 per cent ) of normal volunteers and it was easier to identify the waveform .
	manualset3
90274	6	399038	13	NULL	NULL	0	NULL	97.5 per cent	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when the electrode was placed on the nasal ala , the threshold was significantly lower , an ideal biphasic configuration was present in almost all cases ( 97.5 per cent ) of normal volunteers and it was easier to identify the waveform .
	manualset3
90275	7	399038	13	NULL	NULL	0	NULL	volunteers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when the electrode was placed on the nasal ala , the threshold was significantly lower , an ideal biphasic configuration was present in almost all cases ( 97.5 per cent ) of normal volunteers and it was easier to identify the waveform .
	manualset3
90276	8	399038	13	NULL	NULL	0	NULL	waveform	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when the electrode was placed on the nasal ala , the threshold was significantly lower , an ideal biphasic configuration was present in almost all cases ( 97.5 per cent ) of normal volunteers and it was easier to identify the waveform .
	manualset3
90278	1	399039	13	NULL	NULL	0	NULL	 two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when the two tasks vary randomly from trial to trial , effects of spatial predictability carry over to the perceptual task .
	manualset3
90279	2	399039	13	NULL	NULL	0	NULL	tasks	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when the two tasks vary randomly from trial to trial , effects of spatial predictability carry over to the perceptual task .
	manualset3
90280	3	399039	13	NULL	NULL	0	NULL	trial	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when the two tasks vary randomly from trial to trial , effects of spatial predictability carry over to the perceptual task .
	manualset3
90281	4	399039	13	NULL	NULL	0	NULL	trial 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when the two tasks vary randomly from trial to trial , effects of spatial predictability carry over to the perceptual task .
	manualset3
90282	5	399039	13	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when the two tasks vary randomly from trial to trial , effects of spatial predictability carry over to the perceptual task .
	manualset3
90283	6	399039	13	NULL	NULL	NULL	NULL	spatial predictability	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , when the two tasks vary randomly from trial to trial , effects of spatial predictability carry over to the perceptual task .
	manualset3
90284	7	399039	13	NULL	NULL	0	NULL	task	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when the two tasks vary randomly from trial to trial , effects of spatial predictability carry over to the perceptual task .
	manualset3
90285	1	399040	13	NULL	NULL	0	NULL	depression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , whether depression interferes with the cardioprotection of IPC during myocardial ischemia/reperfusion and their underlying mechanisms remain largely unknown .
	manualset3
90286	2	399040	13	NULL	NULL	NULL	NULL	 cardioprotection of IPC	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , whether depression interferes with the cardioprotection of IPC during myocardial ischemia/reperfusion and their underlying mechanisms remain largely unknown .
	manualset3
90288	4	399040	13	NULL	NULL	0	NULL	myocardial ischemia/reperfusion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , whether depression interferes with the cardioprotection of IPC during myocardial ischemia/reperfusion and their underlying mechanisms remain largely unknown .
	manualset3
90289	5	399040	13	NULL	NULL	0	NULL	mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , whether depression interferes with the cardioprotection of IPC during myocardial ischemia/reperfusion and their underlying mechanisms remain largely unknown .
	manualset3
90290	1	399041	13	NULL	NULL	0	NULL	G ( q ) - PLC pathway 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , whether the G ( q ) - PLC pathway is the main regulator of TRPC4/5 channels and how other G proteins may regulate these channels are poorly understood .
	manualset3
90291	2	399041	13	NULL	NULL	0	NULL	regulator	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , whether the G ( q ) - PLC pathway is the main regulator of TRPC4/5 channels and how other G proteins may regulate these channels are poorly understood .
	manualset3
90292	3	399041	13	NULL	NULL	0	NULL	TRPC4/5 channels	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , whether the G ( q ) - PLC pathway is the main regulator of TRPC4/5 channels and how other G proteins may regulate these channels are poorly understood .
	manualset3
90293	4	399041	13	NULL	NULL	0	NULL	G proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , whether the G ( q ) - PLC pathway is the main regulator of TRPC4/5 channels and how other G proteins may regulate these channels are poorly understood .
	manualset3
90296	5	399041	13	NULL	NULL	0	NULL	channels	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , whether the G ( q ) - PLC pathway is the main regulator of TRPC4/5 channels and how other G proteins may regulate these channels are poorly understood .
	manualset3
90297	1	399042	13	NULL	NULL	0	NULL	specificity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , while the specificity of 4-74-6 is stringent , 2-96-12 cross-reacts with many evolutionarily related cytochromes c. Such a marked difference in specificity of antibodies with overlapping epitopes may represent unique antibody immunodiversity .
	manualset3
90298	2	399042	13	NULL	NULL	0	NULL	4-74-6 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , while the specificity of 4-74-6 is stringent , 2-96-12 cross-reacts with many evolutionarily related cytochromes c. Such a marked difference in specificity of antibodies with overlapping epitopes may represent unique antibody immunodiversity .
	manualset3
90301	3	399042	13	NULL	NULL	0	NULL	2-96-12	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , while the specificity of 4-74-6 is stringent , 2-96-12 cross-reacts with many evolutionarily related cytochromes c. Such a marked difference in specificity of antibodies with overlapping epitopes may represent unique antibody immunodiversity .
	manualset3
90308	4	399042	13	NULL	NULL	0	NULL	cytochromes c	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , while the specificity of 4-74-6 is stringent , 2-96-12 cross-reacts with many evolutionarily related cytochromes c. Such a marked difference in specificity of antibodies with overlapping epitopes may represent unique antibody immunodiversity .
	manualset3
90309	5	399042	13	NULL	NULL	0	NULL	 difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	However , while the specificity of 4-74-6 is stringent , 2-96-12 cross-reacts with many evolutionarily related cytochromes c. Such a marked difference in specificity of antibodies with overlapping epitopes may represent unique antibody immunodiversity .
	manualset3
90311	6	399042	13	NULL	NULL	0	NULL	specificity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , while the specificity of 4-74-6 is stringent , 2-96-12 cross-reacts with many evolutionarily related cytochromes c. Such a marked difference in specificity of antibodies with overlapping epitopes may represent unique antibody immunodiversity .
	manualset3
90312	7	399042	13	NULL	NULL	NULL	NULL	 antibodies	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , while the specificity of 4-74-6 is stringent , 2-96-12 cross-reacts with many evolutionarily related cytochromes c. Such a marked difference in specificity of antibodies with overlapping epitopes may represent unique antibody immunodiversity .
	manualset3
90313	8	399042	13	NULL	NULL	NULL	NULL	 overlapping epitopes	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , while the specificity of 4-74-6 is stringent , 2-96-12 cross-reacts with many evolutionarily related cytochromes c. Such a marked difference in specificity of antibodies with overlapping epitopes may represent unique antibody immunodiversity .
	manualset3
90315	9	399042	13	NULL	NULL	0	NULL	antibody immunodiversity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , while the specificity of 4-74-6 is stringent , 2-96-12 cross-reacts with many evolutionarily related cytochromes c. Such a marked difference in specificity of antibodies with overlapping epitopes may represent unique antibody immunodiversity .
	manualset3
90318	1	399043	13	NULL	NULL	0	NULL	 iron	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	However , why iron accumulates and in what oxidation state iron it accumulates in the brain of PS-exposed rats has not been well elucidated .
	manualset3
90322	2	399043	13	NULL	NULL	NULL	NULL	oxidation state iron	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , why iron accumulates and in what oxidation state iron it accumulates in the brain of PS-exposed rats has not been well elucidated .
	manualset3
90323	3	399043	13	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , why iron accumulates and in what oxidation state iron it accumulates in the brain of PS-exposed rats has not been well elucidated .
	manualset3
90324	4	399043	13	NULL	NULL	0	NULL	PS-exposed rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , why iron accumulates and in what oxidation state iron it accumulates in the brain of PS-exposed rats has not been well elucidated .
	manualset3
90325	1	399044	13	NULL	NULL	0	NULL	improvements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , with the improvements in atherectomy technology , namely plaque excision and laser plaque ablation , the full spectrum of arterial occlusive lesions may now be addressed by percutaneous means with excellent limb salvage rates .
	manualset3
90328	2	399044	13	NULL	NULL	NULL	NULL	atherectomy technology	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , with the improvements in atherectomy technology , namely plaque excision and laser plaque ablation , the full spectrum of arterial occlusive lesions may now be addressed by percutaneous means with excellent limb salvage rates .
	manualset3
90332	3	399044	13	NULL	NULL	0	NULL	plaque excision	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , with the improvements in atherectomy technology , namely plaque excision and laser plaque ablation , the full spectrum of arterial occlusive lesions may now be addressed by percutaneous means with excellent limb salvage rates .
	manualset3
90334	4	399044	13	NULL	NULL	0	NULL	laser plaque ablation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , with the improvements in atherectomy technology , namely plaque excision and laser plaque ablation , the full spectrum of arterial occlusive lesions may now be addressed by percutaneous means with excellent limb salvage rates .
	manualset3
90336	5	399044	13	NULL	NULL	0	NULL	spectrum of arterial occlusive lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , with the improvements in atherectomy technology , namely plaque excision and laser plaque ablation , the full spectrum of arterial occlusive lesions may now be addressed by percutaneous means with excellent limb salvage rates .
	manualset3
90337	6	399044	13	NULL	NULL	0	NULL	limb salvage rates	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , with the improvements in atherectomy technology , namely plaque excision and laser plaque ablation , the full spectrum of arterial occlusive lesions may now be addressed by percutaneous means with excellent limb salvage rates .
	manualset3
91239	7	399044	13	NULL	NULL	NULL	NULL	percutaneous means	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , with the improvements in atherectomy technology , namely plaque excision and laser plaque ablation , the full spectrum of arterial occlusive lesions may now be addressed by percutaneous means with excellent limb salvage rates .
	manualset3
90339	1	399045	13	NULL	NULL	NULL	NULL	 patient	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The patient and the informed consent ) .
	manualset3
90342	2	399045	13	NULL	NULL	NULL	NULL	 informed consent	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The patient and the informed consent ) .
	manualset3
90345	1	399046	13	NULL	NULL	0	NULL	identifications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , with the recent advances in the identifications of unique molecular signatures for CSCs along with ongoing clinical trials targeting CSCs , it is possible to use targeted nanotechnology-based strategies in the management of different types of cancers .
	manualset3
90346	2	399046	13	NULL	NULL	NULL	NULL	unique molecular signatures	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However , with the recent advances in the identifications of unique molecular signatures for CSCs along with ongoing clinical trials targeting CSCs , it is possible to use targeted nanotechnology-based strategies in the management of different types of cancers .
	manualset3
90347	3	399046	13	NULL	NULL	0	NULL	CSCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , with the recent advances in the identifications of unique molecular signatures for CSCs along with ongoing clinical trials targeting CSCs , it is possible to use targeted nanotechnology-based strategies in the management of different types of cancers .
	manualset3
90348	4	399046	13	NULL	NULL	0	NULL	clinical trials targeting CSCs	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , with the recent advances in the identifications of unique molecular signatures for CSCs along with ongoing clinical trials targeting CSCs , it is possible to use targeted nanotechnology-based strategies in the management of different types of cancers .
	manualset3
90349	5	399046	13	NULL	NULL	0	NULL	nanotechnology-based strategies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , with the recent advances in the identifications of unique molecular signatures for CSCs along with ongoing clinical trials targeting CSCs , it is possible to use targeted nanotechnology-based strategies in the management of different types of cancers .
	manualset3
90350	6	399046	13	NULL	NULL	0	NULL	management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , with the recent advances in the identifications of unique molecular signatures for CSCs along with ongoing clinical trials targeting CSCs , it is possible to use targeted nanotechnology-based strategies in the management of different types of cancers .
	manualset3
90351	7	399046	13	NULL	NULL	0	NULL	types of cancers 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	However , with the recent advances in the identifications of unique molecular signatures for CSCs along with ongoing clinical trials targeting CSCs , it is possible to use targeted nanotechnology-based strategies in the management of different types of cancers .
	manualset3
90356	1	399047	13	NULL	NULL	0	NULL	4 ' - O-allyl ether of hygromycin A aglycone 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However a 4 ' - O-allyl ether of hygromycin A aglycone showed an equivalent MIC to hygromycin A , while having a less potent IC50 in the cell free assay .
	manualset3
90357	2	399047	13	NULL	NULL	0	NULL	MIC	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However a 4 ' - O-allyl ether of hygromycin A aglycone showed an equivalent MIC to hygromycin A , while having a less potent IC50 in the cell free assay .
	manualset3
90358	3	399047	13	NULL	NULL	0	NULL	hygromycin A	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However a 4 ' - O-allyl ether of hygromycin A aglycone showed an equivalent MIC to hygromycin A , while having a less potent IC50 in the cell free assay .
	manualset3
90359	4	399047	13	NULL	NULL	0	NULL	 IC50 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However a 4 ' - O-allyl ether of hygromycin A aglycone showed an equivalent MIC to hygromycin A , while having a less potent IC50 in the cell free assay .
	manualset3
90360	5	399047	13	NULL	NULL	0	NULL	cell free assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However a 4 ' - O-allyl ether of hygromycin A aglycone showed an equivalent MIC to hygromycin A , while having a less potent IC50 in the cell free assay .
	manualset3
90361	1	399048	13	NULL	NULL	0	NULL	methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However both methods need very expensive instruments like HPLC and/or Bactec-460 Tb radiometric system .
	manualset3
90362	2	399048	13	NULL	NULL	0	NULL	instruments	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	However both methods need very expensive instruments like HPLC and/or Bactec-460 Tb radiometric system .
	manualset3
90363	3	399048	13	NULL	NULL	0	NULL	HPLC 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However both methods need very expensive instruments like HPLC and/or Bactec-460 Tb radiometric system .
	manualset3
90364	4	399048	13	NULL	NULL	0	NULL	Bactec-460 Tb radiometric system 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	However both methods need very expensive instruments like HPLC and/or Bactec-460 Tb radiometric system .
	manualset3
90365	1	399049	13	NULL	NULL	0	NULL	postoperative pain group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However in the acute postoperative pain group other factors such as depletion of endorphins by drugs used for anesthesia or due to surgical stress can not be excluded .
	manualset3
90366	2	399049	13	NULL	NULL	0	NULL	factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However in the acute postoperative pain group other factors such as depletion of endorphins by drugs used for anesthesia or due to surgical stress can not be excluded .
	manualset3
90367	3	399049	13	NULL	NULL	0	NULL	depletion of endorphins 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However in the acute postoperative pain group other factors such as depletion of endorphins by drugs used for anesthesia or due to surgical stress can not be excluded .
	manualset3
90368	4	399049	13	NULL	NULL	0	NULL	drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However in the acute postoperative pain group other factors such as depletion of endorphins by drugs used for anesthesia or due to surgical stress can not be excluded .
	manualset3
90369	5	399049	13	NULL	NULL	0	NULL	anesthesia	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However in the acute postoperative pain group other factors such as depletion of endorphins by drugs used for anesthesia or due to surgical stress can not be excluded .
	manualset3
90370	6	399049	13	NULL	NULL	0	NULL	 surgical stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However in the acute postoperative pain group other factors such as depletion of endorphins by drugs used for anesthesia or due to surgical stress can not be excluded .
	manualset3
90372	2	399050	13	NULL	NULL	0	NULL	durations 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	However in this study the durations of vecuronium action in patients who required further hemodialysis therapy were also shorter than those during kidney transplantation .
	manualset3
90373	3	399050	13	NULL	NULL	NULL	NULL	vecuronium action	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However in this study the durations of vecuronium action in patients who required further hemodialysis therapy were also shorter than those during kidney transplantation .
	manualset3
90375	5	399050	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However in this study the durations of vecuronium action in patients who required further hemodialysis therapy were also shorter than those during kidney transplantation .
	manualset3
90376	6	399050	13	NULL	NULL	0	NULL	hemodialysis therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However in this study the durations of vecuronium action in patients who required further hemodialysis therapy were also shorter than those during kidney transplantation .
	manualset3
90377	7	399050	13	NULL	NULL	0	NULL	kidney transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However in this study the durations of vecuronium action in patients who required further hemodialysis therapy were also shorter than those during kidney transplantation .
	manualset3
90378	1	399051	13	NULL	NULL	NULL	NULL	non-phosphorylated peptides	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However it can bind to some non-phosphorylated peptides containing one or more aspartic acid residues and/or glutamic acid residues .
	manualset3
90379	2	399051	13	NULL	NULL	0	NULL	one or more aspartic acid residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	However it can bind to some non-phosphorylated peptides containing one or more aspartic acid residues and/or glutamic acid residues .
	manualset3
90380	3	399051	13	NULL	NULL	0	NULL	glutamic acid residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	However it can bind to some non-phosphorylated peptides containing one or more aspartic acid residues and/or glutamic acid residues .
	manualset3
90381	1	399052	13	NULL	NULL	0	NULL	molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However some molecules are able to block in vitro the interaction between a rhinovirus and its receptor : anti-receptor antibodies , soluble ICAM-1 , capsid-binding agents .
	manualset3
90382	2	399052	13	NULL	NULL	0	NULL	 interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However some molecules are able to block in vitro the interaction between a rhinovirus and its receptor : anti-receptor antibodies , soluble ICAM-1 , capsid-binding agents .
	manualset3
90383	3	399052	13	NULL	NULL	0	NULL	rhinovirus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However some molecules are able to block in vitro the interaction between a rhinovirus and its receptor : anti-receptor antibodies , soluble ICAM-1 , capsid-binding agents .
	manualset3
90384	4	399052	13	NULL	NULL	0	NULL	receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However some molecules are able to block in vitro the interaction between a rhinovirus and its receptor : anti-receptor antibodies , soluble ICAM-1 , capsid-binding agents .
	manualset3
90385	5	399052	13	NULL	NULL	0	NULL	anti-receptor antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However some molecules are able to block in vitro the interaction between a rhinovirus and its receptor : anti-receptor antibodies , soluble ICAM-1 , capsid-binding agents .
	manualset3
90386	6	399052	13	NULL	NULL	0	NULL	soluble ICAM-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However some molecules are able to block in vitro the interaction between a rhinovirus and its receptor : anti-receptor antibodies , soluble ICAM-1 , capsid-binding agents .
	manualset3
90389	7	399052	13	NULL	NULL	0	NULL	capsid-binding agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However some molecules are able to block in vitro the interaction between a rhinovirus and its receptor : anti-receptor antibodies , soluble ICAM-1 , capsid-binding agents .
	manualset3
90390	1	399053	13	NULL	NULL	0	NULL	alcoholism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( The present state of alcoholism treatment in Poland ) .
	manualset3
90391	2	399053	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( The present state of alcoholism treatment in Poland ) .
	manualset3
90392	3	399053	13	NULL	NULL	0	NULL	Poland	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( The present state of alcoholism treatment in Poland ) .
	manualset3
90394	5	399053	13	NULL	NULL	0	NULL	state	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The present state of alcoholism treatment in Poland ) .
	manualset3
90395	1	399054	13	NULL	NULL	0	NULL	mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However the mechanism by which AIRE controls gene expression is currently unknown and the function of its domains , in particular of its PHD fingers is still elusive and controversial .
	manualset3
90405	2	399054	13	NULL	NULL	0	NULL	AIRE	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However the mechanism by which AIRE controls gene expression is currently unknown and the function of its domains , in particular of its PHD fingers is still elusive and controversial .
	manualset3
90407	3	399054	13	NULL	NULL	0	NULL	gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However the mechanism by which AIRE controls gene expression is currently unknown and the function of its domains , in particular of its PHD fingers is still elusive and controversial .
	manualset3
90408	4	399054	13	NULL	NULL	0	NULL	 function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However the mechanism by which AIRE controls gene expression is currently unknown and the function of its domains , in particular of its PHD fingers is still elusive and controversial .
	manualset3
90409	5	399054	13	NULL	NULL	0	NULL	domains 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	However the mechanism by which AIRE controls gene expression is currently unknown and the function of its domains , in particular of its PHD fingers is still elusive and controversial .
	manualset3
90410	6	399054	13	NULL	NULL	0	NULL	PHD fingers	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	However the mechanism by which AIRE controls gene expression is currently unknown and the function of its domains , in particular of its PHD fingers is still elusive and controversial .
	manualset3
90414	1	399055	13	NULL	NULL	NULL	NULL	order of activity	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However the order of activity MOR ) MFI ) BEA ) FAU seems to be related to the size of the pores , which may suggest the involvement of a confinement effect in the zeolites cavities .
	manualset3
90415	2	399055	13	NULL	NULL	0	NULL	MOR 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However the order of activity MOR ) MFI ) BEA ) FAU seems to be related to the size of the pores , which may suggest the involvement of a confinement effect in the zeolites cavities .
	manualset3
90417	3	399055	13	NULL	NULL	0	NULL	MFI	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However the order of activity MOR ) MFI ) BEA ) FAU seems to be related to the size of the pores , which may suggest the involvement of a confinement effect in the zeolites cavities .
	manualset3
90418	4	399055	13	NULL	NULL	0	NULL	BEA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However the order of activity MOR ) MFI ) BEA ) FAU seems to be related to the size of the pores , which may suggest the involvement of a confinement effect in the zeolites cavities .
	manualset3
90419	5	399055	13	NULL	NULL	0	NULL	FAU 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However the order of activity MOR ) MFI ) BEA ) FAU seems to be related to the size of the pores , which may suggest the involvement of a confinement effect in the zeolites cavities .
	manualset3
90421	6	399055	13	NULL	NULL	0	NULL	size of the pores	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	However the order of activity MOR ) MFI ) BEA ) FAU seems to be related to the size of the pores , which may suggest the involvement of a confinement effect in the zeolites cavities .
	manualset3
90424	7	399055	13	NULL	NULL	0	NULL	involvement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However the order of activity MOR ) MFI ) BEA ) FAU seems to be related to the size of the pores , which may suggest the involvement of a confinement effect in the zeolites cavities .
	manualset3
90425	8	399055	13	NULL	NULL	0	NULL	confinement effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However the order of activity MOR ) MFI ) BEA ) FAU seems to be related to the size of the pores , which may suggest the involvement of a confinement effect in the zeolites cavities .
	manualset3
90427	9	399055	13	NULL	NULL	0	NULL	zeolites cavities	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	However the order of activity MOR ) MFI ) BEA ) FAU seems to be related to the size of the pores , which may suggest the involvement of a confinement effect in the zeolites cavities .
	manualset3
90473	1	399056	13	NULL	NULL	NULL	NULL	hyponatremia warrant	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However the potentially severe affects of hyponatremia warrant close monitoring of these patients and the establishment of methods to prevent this problem from occurring .
	manualset3
90475	3	399056	13	NULL	NULL	0	NULL	monitoring	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However the potentially severe affects of hyponatremia warrant close monitoring of these patients and the establishment of methods to prevent this problem from occurring .
	manualset3
90476	4	399056	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However the potentially severe affects of hyponatremia warrant close monitoring of these patients and the establishment of methods to prevent this problem from occurring .
	manualset3
90477	5	399056	13	NULL	NULL	0	NULL	 establishment of methods 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However the potentially severe affects of hyponatremia warrant close monitoring of these patients and the establishment of methods to prevent this problem from occurring .
	manualset3
91076	6	399056	13	NULL	NULL	0	NULL	problem	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However the potentially severe affects of hyponatremia warrant close monitoring of these patients and the establishment of methods to prevent this problem from occurring .
	manualset3
90478	1	399057	13	NULL	NULL	0	NULL	HoxB5 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	HoxB5 mRNA colocalized with flk1 expression in differentiating embryoid bodies , and HoxB5 potently transactivated the flk1 promoter in an HBE-dependent fashion in transient-transfection assays .
	manualset3
90479	2	399057	13	NULL	NULL	0	NULL	flk1 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HoxB5 mRNA colocalized with flk1 expression in differentiating embryoid bodies , and HoxB5 potently transactivated the flk1 promoter in an HBE-dependent fashion in transient-transfection assays .
	manualset3
90480	3	399057	13	NULL	NULL	0	NULL	embryoid bodies	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	HoxB5 mRNA colocalized with flk1 expression in differentiating embryoid bodies , and HoxB5 potently transactivated the flk1 promoter in an HBE-dependent fashion in transient-transfection assays .
	manualset3
90481	4	399057	13	NULL	NULL	0	NULL	HoxB5 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	HoxB5 mRNA colocalized with flk1 expression in differentiating embryoid bodies , and HoxB5 potently transactivated the flk1 promoter in an HBE-dependent fashion in transient-transfection assays .
	manualset3
90482	5	399057	13	NULL	NULL	0	NULL	flk1 promoter 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	HoxB5 mRNA colocalized with flk1 expression in differentiating embryoid bodies , and HoxB5 potently transactivated the flk1 promoter in an HBE-dependent fashion in transient-transfection assays .
	manualset3
90483	6	399057	13	NULL	NULL	0	NULL	HBE-dependent fashion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HoxB5 mRNA colocalized with flk1 expression in differentiating embryoid bodies , and HoxB5 potently transactivated the flk1 promoter in an HBE-dependent fashion in transient-transfection assays .
	manualset3
90484	7	399057	13	NULL	NULL	0	NULL	transient-transfection assays 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	HoxB5 mRNA colocalized with flk1 expression in differentiating embryoid bodies , and HoxB5 potently transactivated the flk1 promoter in an HBE-dependent fashion in transient-transfection assays .
	manualset3
90485	1	399058	13	NULL	NULL	0	NULL	Hp	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hp administrated orally along with Cd injection for 21 days , significantly revert back the status of oxidative stress markers , Cd concentration in testis , improved status of antioxidant markers and membrane bound enzymes in the testis to near normal level .
	manualset3
90486	2	399058	13	NULL	NULL	0	NULL	Cd injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hp administrated orally along with Cd injection for 21 days , significantly revert back the status of oxidative stress markers , Cd concentration in testis , improved status of antioxidant markers and membrane bound enzymes in the testis to near normal level .
	manualset3
90487	3	399058	13	NULL	NULL	0	NULL	21 days	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Hp administrated orally along with Cd injection for 21 days , significantly revert back the status of oxidative stress markers , Cd concentration in testis , improved status of antioxidant markers and membrane bound enzymes in the testis to near normal level .
	manualset3
90488	4	399058	13	NULL	NULL	0	NULL	 status of oxidative stress markers	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hp administrated orally along with Cd injection for 21 days , significantly revert back the status of oxidative stress markers , Cd concentration in testis , improved status of antioxidant markers and membrane bound enzymes in the testis to near normal level .
	manualset3
90489	5	399058	13	NULL	NULL	0	NULL	Cd concentration in testis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hp administrated orally along with Cd injection for 21 days , significantly revert back the status of oxidative stress markers , Cd concentration in testis , improved status of antioxidant markers and membrane bound enzymes in the testis to near normal level .
	manualset3
90490	6	399058	13	NULL	NULL	0	NULL	status of antioxidant markers	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hp administrated orally along with Cd injection for 21 days , significantly revert back the status of oxidative stress markers , Cd concentration in testis , improved status of antioxidant markers and membrane bound enzymes in the testis to near normal level .
	manualset3
90491	7	399058	13	NULL	NULL	0	NULL	membrane bound enzymes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hp administrated orally along with Cd injection for 21 days , significantly revert back the status of oxidative stress markers , Cd concentration in testis , improved status of antioxidant markers and membrane bound enzymes in the testis to near normal level .
	manualset3
90492	8	399058	13	NULL	NULL	0	NULL	testis 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Hp administrated orally along with Cd injection for 21 days , significantly revert back the status of oxidative stress markers , Cd concentration in testis , improved status of antioxidant markers and membrane bound enzymes in the testis to near normal level .
	manualset3
90493	9	399058	13	NULL	NULL	0	NULL	level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hp administrated orally along with Cd injection for 21 days , significantly revert back the status of oxidative stress markers , Cd concentration in testis , improved status of antioxidant markers and membrane bound enzymes in the testis to near normal level .
	manualset3
90494	1	399059	13	NULL	NULL	0	NULL	Hsp70	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hsp70 was strongly induced in all exposure groups , which also included bisphenol A and diallylphthalate .
	manualset3
90495	2	399059	13	NULL	NULL	0	NULL	exposure groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hsp70 was strongly induced in all exposure groups , which also included bisphenol A and diallylphthalate .
	manualset3
90496	3	399059	13	NULL	NULL	0	NULL	bisphenol A	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hsp70 was strongly induced in all exposure groups , which also included bisphenol A and diallylphthalate .
	manualset3
90497	4	399059	13	NULL	NULL	0	NULL	 diallylphthalate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hsp70 was strongly induced in all exposure groups , which also included bisphenol A and diallylphthalate .
	manualset3
90498	1	399060	13	NULL	NULL	0	NULL	Human B cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Human B cells express two closely related immunoglobulin G receptors , FcRIIb1 and FcRIIb2 , which differ by a 19 amino acid insertion in the cytoplasmic tail of FcRIIb1 .
	manualset3
90499	2	399060	13	NULL	NULL	0	NULL	two 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Human B cells express two closely related immunoglobulin G receptors , FcRIIb1 and FcRIIb2 , which differ by a 19 amino acid insertion in the cytoplasmic tail of FcRIIb1 .
	manualset3
90500	3	399060	13	NULL	NULL	0	NULL	immunoglobulin G receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Human B cells express two closely related immunoglobulin G receptors , FcRIIb1 and FcRIIb2 , which differ by a 19 amino acid insertion in the cytoplasmic tail of FcRIIb1 .
	manualset3
90501	4	399060	13	NULL	NULL	0	NULL	FcRIIb1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human B cells express two closely related immunoglobulin G receptors , FcRIIb1 and FcRIIb2 , which differ by a 19 amino acid insertion in the cytoplasmic tail of FcRIIb1 .
	manualset3
90502	5	399060	13	NULL	NULL	0	NULL	FcRIIb2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human B cells express two closely related immunoglobulin G receptors , FcRIIb1 and FcRIIb2 , which differ by a 19 amino acid insertion in the cytoplasmic tail of FcRIIb1 .
	manualset3
90503	6	399060	13	NULL	NULL	0	NULL	19 amino acid insertion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Human B cells express two closely related immunoglobulin G receptors , FcRIIb1 and FcRIIb2 , which differ by a 19 amino acid insertion in the cytoplasmic tail of FcRIIb1 .
	manualset3
90504	7	399060	13	NULL	NULL	0	NULL	cytoplasmic tail of FcRIIb1 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human B cells express two closely related immunoglobulin G receptors , FcRIIb1 and FcRIIb2 , which differ by a 19 amino acid insertion in the cytoplasmic tail of FcRIIb1 .
	manualset3
90505	1	399061	13	NULL	NULL	0	NULL	Human CysC	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human CysC also increased the number of neurospheres formed from embryonic brain , and thus it increases the number of neural stem/precursor cells in a manner similar to glycosylated rat CysC .
	manualset3
90506	2	399061	13	NULL	NULL	NULL	NULL	number of neurospheres	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human CysC also increased the number of neurospheres formed from embryonic brain , and thus it increases the number of neural stem/precursor cells in a manner similar to glycosylated rat CysC .
	manualset3
90507	3	399061	13	NULL	NULL	0	NULL	embryonic brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Human CysC also increased the number of neurospheres formed from embryonic brain , and thus it increases the number of neural stem/precursor cells in a manner similar to glycosylated rat CysC .
	manualset3
90508	4	399061	13	NULL	NULL	NULL	NULL	number of neural stem/precursor cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human CysC also increased the number of neurospheres formed from embryonic brain , and thus it increases the number of neural stem/precursor cells in a manner similar to glycosylated rat CysC .
	manualset3
90509	5	399061	13	NULL	NULL	0	NULL	glycosylated rat CysC	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human CysC also increased the number of neurospheres formed from embryonic brain , and thus it increases the number of neural stem/precursor cells in a manner similar to glycosylated rat CysC .
	manualset3
90510	1	399062	13	NULL	NULL	0	NULL	Human Cytomegalovirus ( HCMV ) infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Human Cytomegalovirus ( HCMV ) infection induces several metabolic activities that have been found to be important for viral replication .
	manualset3
90511	2	399062	13	NULL	NULL	NULL	NULL	metabolic activities 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human Cytomegalovirus ( HCMV ) infection induces several metabolic activities that have been found to be important for viral replication .
	manualset3
90512	3	399062	13	NULL	NULL	0	NULL	viral replication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Human Cytomegalovirus ( HCMV ) infection induces several metabolic activities that have been found to be important for viral replication .
	manualset3
90513	1	399063	13	NULL	NULL	0	NULL	Human EEG activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Human EEG activity in the conventional frequency range of 1-30 c/s is a well-established entity .
	manualset3
90514	2	399063	13	NULL	NULL	0	NULL	frequency range	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Human EEG activity in the conventional frequency range of 1-30 c/s is a well-established entity .
	manualset3
90515	3	399063	13	NULL	NULL	0	NULL	1-30 c/s 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Human EEG activity in the conventional frequency range of 1-30 c/s is a well-established entity .
	manualset3
90516	4	399063	13	NULL	NULL	NULL	NULL	well-established entity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human EEG activity in the conventional frequency range of 1-30 c/s is a well-established entity .
	manualset3
90517	1	399064	13	NULL	NULL	0	NULL	 problem of cervical ribs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( The problem of cervical ribs in internal medicine ) .
	manualset3
90518	2	399064	13	NULL	NULL	NULL	NULL	internal medicine	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The problem of cervical ribs in internal medicine ) .
	manualset3
90519	1	399065	13	NULL	NULL	0	NULL	Human Immunodeficiency virus type 1 Nef	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human Immunodeficiency virus type 1 Nef potently induces apoptosis in primary human brain microvascular endothelial cells via the activation of caspases .
	manualset3
90520	2	399065	13	NULL	NULL	NULL	NULL	apoptosis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human Immunodeficiency virus type 1 Nef potently induces apoptosis in primary human brain microvascular endothelial cells via the activation of caspases .
	manualset3
90521	3	399065	13	NULL	NULL	0	NULL	primary human brain microvascular endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Human Immunodeficiency virus type 1 Nef potently induces apoptosis in primary human brain microvascular endothelial cells via the activation of caspases .
	manualset3
90522	4	399065	13	NULL	NULL	0	NULL	activation of caspases	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Human Immunodeficiency virus type 1 Nef potently induces apoptosis in primary human brain microvascular endothelial cells via the activation of caspases .
	manualset3
90523	1	399066	13	NULL	NULL	0	NULL	Human LDL 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human LDL was oxidized in the presence of CuSO ( 4 ) ( ox-LDL ) .
	manualset3
90524	2	399066	13	NULL	NULL	0	NULL	 CuSO ( 4 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Human LDL was oxidized in the presence of CuSO ( 4 ) ( ox-LDL ) .
	manualset3
90525	3	399066	13	NULL	NULL	0	NULL	ox-LDL 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human LDL was oxidized in the presence of CuSO ( 4 ) ( ox-LDL ) .
	manualset3
90526	1	399067	13	NULL	NULL	0	NULL	Human NEIL2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human NEIL2 , one of five oxidized base-specific DNA glycosylases , is unique in preferentially repairing oxidative damage in transcribed genes .
	manualset3
90527	2	399067	13	NULL	NULL	0	NULL	one of five oxidized base-specific DNA glycosylases	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human NEIL2 , one of five oxidized base-specific DNA glycosylases , is unique in preferentially repairing oxidative damage in transcribed genes .
	manualset3
90528	3	399067	13	NULL	NULL	NULL	NULL	oxidative damage 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human NEIL2 , one of five oxidized base-specific DNA glycosylases , is unique in preferentially repairing oxidative damage in transcribed genes .
	manualset3
90529	4	399067	13	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Human NEIL2 , one of five oxidized base-specific DNA glycosylases , is unique in preferentially repairing oxidative damage in transcribed genes .
	manualset3
90530	1	399068	13	NULL	NULL	0	NULL	Human P450c17	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human P450c17 is expressed in a cAMP-responsive , cell-specific , developmentally programmed fashion , but little is known about its transcriptional regulation .
	manualset3
90531	2	399068	13	NULL	NULL	NULL	NULL	cAMP-responsive fashion	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human P450c17 is expressed in a cAMP-responsive , cell-specific , developmentally programmed fashion , but little is known about its transcriptional regulation .
	manualset3
90532	3	399068	13	NULL	NULL	NULL	NULL	cell-specific fashion	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human P450c17 is expressed in a cAMP-responsive , cell-specific , developmentally programmed fashion , but little is known about its transcriptional regulation .
	manualset3
90533	4	399068	13	NULL	NULL	NULL	NULL	developmentally programmed fashion	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human P450c17 is expressed in a cAMP-responsive , cell-specific , developmentally programmed fashion , but little is known about its transcriptional regulation .
	manualset3
90534	5	399068	13	NULL	NULL	0	NULL	 transcriptional regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Human P450c17 is expressed in a cAMP-responsive , cell-specific , developmentally programmed fashion , but little is known about its transcriptional regulation .
	manualset3
90535	1	399069	13	NULL	NULL	0	NULL	Human RhAG ammonia channel	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human RhAG ammonia channel is impaired by the Phe65Ser mutation in overhydrated stomatocytic red cells .
	manualset3
90536	2	399069	13	NULL	NULL	0	NULL	Phe65Ser mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Human RhAG ammonia channel is impaired by the Phe65Ser mutation in overhydrated stomatocytic red cells .
	manualset3
90537	3	399069	13	NULL	NULL	0	NULL	stomatocytic red cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Human RhAG ammonia channel is impaired by the Phe65Ser mutation in overhydrated stomatocytic red cells .
	manualset3
90538	1	399070	13	NULL	NULL	0	NULL	Human atrial natriuretic factor ( ANF ) levels 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Human atrial natriuretic factor ( ANF ) levels were measured before and after peritoneovenous shunt implantation in 10 cirrhotic patients with ascites , in whom sodium retention is a major clinical problem .
	manualset3
90539	2	399070	13	NULL	NULL	0	NULL	 peritoneovenous shunt implantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Human atrial natriuretic factor ( ANF ) levels were measured before and after peritoneovenous shunt implantation in 10 cirrhotic patients with ascites , in whom sodium retention is a major clinical problem .
	manualset3
90540	3	399070	13	NULL	NULL	0	NULL	10 cirrhotic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Human atrial natriuretic factor ( ANF ) levels were measured before and after peritoneovenous shunt implantation in 10 cirrhotic patients with ascites , in whom sodium retention is a major clinical problem .
	manualset3
90541	4	399070	13	NULL	NULL	0	NULL	ascites	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Human atrial natriuretic factor ( ANF ) levels were measured before and after peritoneovenous shunt implantation in 10 cirrhotic patients with ascites , in whom sodium retention is a major clinical problem .
	manualset3
90542	5	399070	13	NULL	NULL	0	NULL	sodium retention	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Human atrial natriuretic factor ( ANF ) levels were measured before and after peritoneovenous shunt implantation in 10 cirrhotic patients with ascites , in whom sodium retention is a major clinical problem .
	manualset3
90543	6	399070	13	NULL	NULL	NULL	NULL	major clinical problem 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human atrial natriuretic factor ( ANF ) levels were measured before and after peritoneovenous shunt implantation in 10 cirrhotic patients with ascites , in whom sodium retention is a major clinical problem .
	manualset3
90544	1	399071	13	NULL	NULL	0	NULL	Human calmodulin	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Human calmodulin is encoded by three genes CALM1 , CALM2 and CALM3 located on different chromosomes .
	manualset3
90545	2	399071	13	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Human calmodulin is encoded by three genes CALM1 , CALM2 and CALM3 located on different chromosomes .
	manualset3
90546	3	399071	13	NULL	NULL	NULL	NULL	genes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human calmodulin is encoded by three genes CALM1 , CALM2 and CALM3 located on different chromosomes .
	manualset3
90547	4	399071	13	NULL	NULL	0	NULL	CALM1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Human calmodulin is encoded by three genes CALM1 , CALM2 and CALM3 located on different chromosomes .
	manualset3
90548	5	399071	13	NULL	NULL	0	NULL	CALM2	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Human calmodulin is encoded by three genes CALM1 , CALM2 and CALM3 located on different chromosomes .
	manualset3
90549	6	399071	13	NULL	NULL	0	NULL	CALM3 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Human calmodulin is encoded by three genes CALM1 , CALM2 and CALM3 located on different chromosomes .
	manualset3
90550	7	399071	13	NULL	NULL	0	NULL	chromosomes 	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Human calmodulin is encoded by three genes CALM1 , CALM2 and CALM3 located on different chromosomes .
	manualset3
90551	1	399072	13	NULL	NULL	0	NULL	Human carboxypeptidase D ( CPD )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human carboxypeptidase D ( CPD ) is a 180-kDa type I membrane protein with three tandem active site domains .
	manualset3
90552	2	399072	13	NULL	NULL	0	NULL	180-kDa type I membrane protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human carboxypeptidase D ( CPD ) is a 180-kDa type I membrane protein with three tandem active site domains .
	manualset3
90553	3	399072	13	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Human carboxypeptidase D ( CPD ) is a 180-kDa type I membrane protein with three tandem active site domains .
	manualset3
90554	4	399072	13	NULL	NULL	0	NULL	tandem active site domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human carboxypeptidase D ( CPD ) is a 180-kDa type I membrane protein with three tandem active site domains .
	manualset3
90555	1	399073	13	NULL	NULL	NULL	NULL	Human cerebellar hypoplasia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human cerebellar hypoplasia : a syndrome of diverse causes .
	manualset3
90556	2	399073	13	NULL	NULL	0	NULL	syndrome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Human cerebellar hypoplasia : a syndrome of diverse causes .
	manualset3
90557	3	399073	13	NULL	NULL	0	NULL	causes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Human cerebellar hypoplasia : a syndrome of diverse causes .
	manualset3
90558	1	399074	13	NULL	NULL	NULL	NULL	problem of individuality	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The problem of individuality in taxonomy ) .
	manualset3
90559	2	399074	13	NULL	NULL	0	NULL	taxonomy	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( The problem of individuality in taxonomy ) .
	manualset3
90560	1	399075	13	NULL	NULL	0	NULL	Human chondrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Human chondrocytes that overexpressed IL-1RII were resistant to IL-1-induced IL-1beta mRNA accumulation and inhibition of proteoglycan synthesis .
	manualset3
90561	2	399075	13	NULL	NULL	0	NULL	 IL-1RII	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human chondrocytes that overexpressed IL-1RII were resistant to IL-1-induced IL-1beta mRNA accumulation and inhibition of proteoglycan synthesis .
	manualset3
90562	3	399075	13	NULL	NULL	0	NULL	IL-1-induced IL-1beta mRNA accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Human chondrocytes that overexpressed IL-1RII were resistant to IL-1-induced IL-1beta mRNA accumulation and inhibition of proteoglycan synthesis .
	manualset3
90563	4	399075	13	NULL	NULL	0	NULL	inhibition of proteoglycan synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Human chondrocytes that overexpressed IL-1RII were resistant to IL-1-induced IL-1beta mRNA accumulation and inhibition of proteoglycan synthesis .
	manualset3
90564	1	399076	13	NULL	NULL	0	NULL	Human chorionic gonadotropin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human chorionic gonadotropin in lung and lung tumors .
	manualset3
90565	2	399076	13	NULL	NULL	0	NULL	lung	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Human chorionic gonadotropin in lung and lung tumors .
	manualset3
90566	3	399076	13	NULL	NULL	0	NULL	lung tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Human chorionic gonadotropin in lung and lung tumors .
	manualset3
90567	1	399077	13	NULL	NULL	0	NULL	Human chorionic gonadotropin levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Human chorionic gonadotropin levels were 33.25-174315 .5 IU/l .
	manualset3
90568	2	399077	13	NULL	NULL	0	NULL	33.25-174315 .5 IU/l	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Human chorionic gonadotropin levels were 33.25-174315 .5 IU/l .
	manualset3
90569	1	399078	13	NULL	NULL	0	NULL	Human eIF4AIII 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human eIF4AIII interacts with an eIF4G-like partner , NOM1 , revealing an evolutionarily conserved function outside the exon junction complex .
	manualset3
90570	2	399078	13	NULL	NULL	0	NULL	eIF4G-like partner	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human eIF4AIII interacts with an eIF4G-like partner , NOM1 , revealing an evolutionarily conserved function outside the exon junction complex .
	manualset3
90571	3	399078	13	NULL	NULL	0	NULL	NOM1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human eIF4AIII interacts with an eIF4G-like partner , NOM1 , revealing an evolutionarily conserved function outside the exon junction complex .
	manualset3
90572	4	399078	13	NULL	NULL	0	NULL	function 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Human eIF4AIII interacts with an eIF4G-like partner , NOM1 , revealing an evolutionarily conserved function outside the exon junction complex .
	manualset3
90573	5	399078	13	NULL	NULL	0	NULL	exon junction complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Human eIF4AIII interacts with an eIF4G-like partner , NOM1 , revealing an evolutionarily conserved function outside the exon junction complex .
	manualset3
90574	1	399079	13	NULL	NULL	0	NULL	Human enhancer of invasion-cluster ( HEI-C )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human enhancer of invasion-cluster ( HEI-C ) , encoding a novel evolutionarily conserved coiled-coil protein , was isolated in a screen for human genes that induce agar invasion in S. cerevisiae .
	manualset3
90575	2	399079	13	NULL	NULL	0	NULL	 coiled-coil protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human enhancer of invasion-cluster ( HEI-C ) , encoding a novel evolutionarily conserved coiled-coil protein , was isolated in a screen for human genes that induce agar invasion in S. cerevisiae .
	manualset3
90576	3	399079	13	NULL	NULL	0	NULL	screen	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Human enhancer of invasion-cluster ( HEI-C ) , encoding a novel evolutionarily conserved coiled-coil protein , was isolated in a screen for human genes that induce agar invasion in S. cerevisiae .
	manualset3
90577	4	399079	13	NULL	NULL	0	NULL	human genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Human enhancer of invasion-cluster ( HEI-C ) , encoding a novel evolutionarily conserved coiled-coil protein , was isolated in a screen for human genes that induce agar invasion in S. cerevisiae .
	manualset3
90578	5	399079	13	NULL	NULL	0	NULL	agar invasion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Human enhancer of invasion-cluster ( HEI-C ) , encoding a novel evolutionarily conserved coiled-coil protein , was isolated in a screen for human genes that induce agar invasion in S. cerevisiae .
	manualset3
90579	6	399079	13	NULL	NULL	0	NULL	S. cerevisiae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Human enhancer of invasion-cluster ( HEI-C ) , encoding a novel evolutionarily conserved coiled-coil protein , was isolated in a screen for human genes that induce agar invasion in S. cerevisiae .
	manualset3
90580	1	399080	13	NULL	NULL	0	NULL	Human fibrinogen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human fibrinogen specifically binds hyaluronic acid .
	manualset3
90581	2	399080	13	NULL	NULL	0	NULL	hyaluronic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Human fibrinogen specifically binds hyaluronic acid .
	manualset3
90582	1	399081	13	NULL	NULL	0	NULL	Human fibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Human fibroblasts were cultured in the absence and presence of cadmium sulfide nanoparticles to evaluate cytotoxicity and cell compatibility .
	manualset3
90583	2	399081	13	NULL	NULL	NULL	NULL	 presence of cadmium sulfide nanoparticles	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human fibroblasts were cultured in the absence and presence of cadmium sulfide nanoparticles to evaluate cytotoxicity and cell compatibility .
	manualset3
90584	3	399081	13	NULL	NULL	NULL	NULL	absence of cadmium sulfide nanoparticles 	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human fibroblasts were cultured in the absence and presence of cadmium sulfide nanoparticles to evaluate cytotoxicity and cell compatibility .
	manualset3
90586	5	399081	13	NULL	NULL	0	NULL	 cytotoxicity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Human fibroblasts were cultured in the absence and presence of cadmium sulfide nanoparticles to evaluate cytotoxicity and cell compatibility .
	manualset3
90587	6	399081	13	NULL	NULL	0	NULL	cell compatibility	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Human fibroblasts were cultured in the absence and presence of cadmium sulfide nanoparticles to evaluate cytotoxicity and cell compatibility .
	manualset3
90588	1	399082	13	NULL	NULL	0	NULL	Human gyrovirus DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Human gyrovirus DNA in human blood , Italy .
	manualset3
90589	2	399082	13	NULL	NULL	0	NULL	human blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Human gyrovirus DNA in human blood , Italy .
	manualset3
90590	3	399082	13	NULL	NULL	0	NULL	 Italy	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Human gyrovirus DNA in human blood , Italy .
	manualset3
90591	1	399083	13	NULL	NULL	0	NULL	Human infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Human infants use prosodic cues present in speech to extract language regularities , and it has been suggested that this capacity is anchored in more general mechanisms that are shared across mammals .
	manualset3
90592	2	399083	13	NULL	NULL	NULL	NULL	prosodic cues 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human infants use prosodic cues present in speech to extract language regularities , and it has been suggested that this capacity is anchored in more general mechanisms that are shared across mammals .
	manualset3
90593	3	399083	13	NULL	NULL	0	NULL	speech 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Human infants use prosodic cues present in speech to extract language regularities , and it has been suggested that this capacity is anchored in more general mechanisms that are shared across mammals .
	manualset3
90594	4	399083	13	NULL	NULL	0	NULL	 language regularities	Language												NULL		0	NULL	NULL	NULL	NULL	NULL	Human infants use prosodic cues present in speech to extract language regularities , and it has been suggested that this capacity is anchored in more general mechanisms that are shared across mammals .
	manualset3
90595	5	399083	13	NULL	NULL	0	NULL	capacity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Human infants use prosodic cues present in speech to extract language regularities , and it has been suggested that this capacity is anchored in more general mechanisms that are shared across mammals .
	manualset3
90596	6	399083	13	NULL	NULL	0	NULL	mechanisms 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Human infants use prosodic cues present in speech to extract language regularities , and it has been suggested that this capacity is anchored in more general mechanisms that are shared across mammals .
	manualset3
90597	7	399083	13	NULL	NULL	0	NULL	mammals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Human infants use prosodic cues present in speech to extract language regularities , and it has been suggested that this capacity is anchored in more general mechanisms that are shared across mammals .
	manualset3
90598	1	399084	13	NULL	NULL	0	NULL	Human leukocyte antigen-G ( HLA-G )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Human leukocyte antigen-G ( HLA-G ) is an MHC class I gene of particular interest in reproductive biology because of its specific expression on fetal cytotrophoblast cells , and its reported involvement both in protection of the developing fetus from destruction by the maternal immune response and in the prevention of maternal pre-eclampsia .
	manualset3
90599	2	399084	13	NULL	NULL	0	NULL	 MHC class I gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Human leukocyte antigen-G ( HLA-G ) is an MHC class I gene of particular interest in reproductive biology because of its specific expression on fetal cytotrophoblast cells , and its reported involvement both in protection of the developing fetus from destruction by the maternal immune response and in the prevention of maternal pre-eclampsia .
	manualset3
90600	3	399084	13	NULL	NULL	0	NULL	reproductive biology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Human leukocyte antigen-G ( HLA-G ) is an MHC class I gene of particular interest in reproductive biology because of its specific expression on fetal cytotrophoblast cells , and its reported involvement both in protection of the developing fetus from destruction by the maternal immune response and in the prevention of maternal pre-eclampsia .
	manualset3
90601	4	399084	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Human leukocyte antigen-G ( HLA-G ) is an MHC class I gene of particular interest in reproductive biology because of its specific expression on fetal cytotrophoblast cells , and its reported involvement both in protection of the developing fetus from destruction by the maternal immune response and in the prevention of maternal pre-eclampsia .
	manualset3
90602	5	399084	13	NULL	NULL	0	NULL	fetal cytotrophoblast cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Human leukocyte antigen-G ( HLA-G ) is an MHC class I gene of particular interest in reproductive biology because of its specific expression on fetal cytotrophoblast cells , and its reported involvement both in protection of the developing fetus from destruction by the maternal immune response and in the prevention of maternal pre-eclampsia .
	manualset3
90603	6	399084	13	NULL	NULL	NULL	NULL	involvement	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human leukocyte antigen-G ( HLA-G ) is an MHC class I gene of particular interest in reproductive biology because of its specific expression on fetal cytotrophoblast cells , and its reported involvement both in protection of the developing fetus from destruction by the maternal immune response and in the prevention of maternal pre-eclampsia .
	manualset3
90604	7	399084	13	NULL	NULL	0	NULL	protection 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Human leukocyte antigen-G ( HLA-G ) is an MHC class I gene of particular interest in reproductive biology because of its specific expression on fetal cytotrophoblast cells , and its reported involvement both in protection of the developing fetus from destruction by the maternal immune response and in the prevention of maternal pre-eclampsia .
	manualset3
90605	8	399084	13	NULL	NULL	NULL	NULL	developing fetus 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human leukocyte antigen-G ( HLA-G ) is an MHC class I gene of particular interest in reproductive biology because of its specific expression on fetal cytotrophoblast cells , and its reported involvement both in protection of the developing fetus from destruction by the maternal immune response and in the prevention of maternal pre-eclampsia .
	manualset3
90606	9	399084	13	NULL	NULL	NULL	NULL	destruction	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human leukocyte antigen-G ( HLA-G ) is an MHC class I gene of particular interest in reproductive biology because of its specific expression on fetal cytotrophoblast cells , and its reported involvement both in protection of the developing fetus from destruction by the maternal immune response and in the prevention of maternal pre-eclampsia .
	manualset3
90607	10	399084	13	NULL	NULL	NULL	NULL	maternal immune response 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human leukocyte antigen-G ( HLA-G ) is an MHC class I gene of particular interest in reproductive biology because of its specific expression on fetal cytotrophoblast cells , and its reported involvement both in protection of the developing fetus from destruction by the maternal immune response and in the prevention of maternal pre-eclampsia .
	manualset3
90608	11	399084	13	NULL	NULL	NULL	NULL	prevention 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human leukocyte antigen-G ( HLA-G ) is an MHC class I gene of particular interest in reproductive biology because of its specific expression on fetal cytotrophoblast cells , and its reported involvement both in protection of the developing fetus from destruction by the maternal immune response and in the prevention of maternal pre-eclampsia .
	manualset3
90609	12	399084	13	NULL	NULL	NULL	NULL	maternal pre-eclampsia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human leukocyte antigen-G ( HLA-G ) is an MHC class I gene of particular interest in reproductive biology because of its specific expression on fetal cytotrophoblast cells , and its reported involvement both in protection of the developing fetus from destruction by the maternal immune response and in the prevention of maternal pre-eclampsia .
	manualset3
90610	1	399085	13	NULL	NULL	0	NULL	production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The production of alcohol and the growth rate of baker 's yeast cultivated in the presence of air ) .
	manualset3
90611	2	399085	13	NULL	NULL	0	NULL	alcohol 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	( The production of alcohol and the growth rate of baker 's yeast cultivated in the presence of air ) .
	manualset3
90612	3	399085	13	NULL	NULL	0	NULL	growth rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( The production of alcohol and the growth rate of baker 's yeast cultivated in the presence of air ) .
	manualset3
90613	4	399085	13	NULL	NULL	0	NULL	baker 's yeast	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( The production of alcohol and the growth rate of baker 's yeast cultivated in the presence of air ) .
	manualset3
90614	5	399085	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The production of alcohol and the growth rate of baker 's yeast cultivated in the presence of air ) .
	manualset3
90615	6	399085	13	NULL	NULL	0	NULL	air	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	( The production of alcohol and the growth rate of baker 's yeast cultivated in the presence of air ) .
	manualset3
90739	1	399086	13	NULL	NULL	0	NULL	Human long-term bone marrow cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Human long-term bone marrow cultures allow persistence of hematopoietic stem cells in vitro for several weeks .
	manualset3
90740	2	399086	13	NULL	NULL	0	NULL	persistence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Human long-term bone marrow cultures allow persistence of hematopoietic stem cells in vitro for several weeks .
	manualset3
90741	3	399086	13	NULL	NULL	0	NULL	hematopoietic stem cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Human long-term bone marrow cultures allow persistence of hematopoietic stem cells in vitro for several weeks .
	manualset3
90742	4	399086	13	NULL	NULL	NULL	NULL	several weeks	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human long-term bone marrow cultures allow persistence of hematopoietic stem cells in vitro for several weeks .
	manualset3
90743	1	399087	13	NULL	NULL	0	NULL	Human malignant T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Human malignant T cells capable of inducing an immunoglobulin class switch .
	manualset3
90745	3	399087	13	NULL	NULL	NULL	NULL	 immunoglobulin class switch	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human malignant T cells capable of inducing an immunoglobulin class switch .
	manualset3
90746	1	399088	13	NULL	NULL	0	NULL	Human monocyte-derived macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Human monocyte-derived macrophages treated with recombinant IFN-gamma ( rIFN-gamma ) and control cells were assessed for three distinct effector functions , all mediated by Fc receptors .
	manualset3
90749	2	399088	13	NULL	NULL	0	NULL	recombinant IFN-gamma ( rIFN-gamma )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human monocyte-derived macrophages treated with recombinant IFN-gamma ( rIFN-gamma ) and control cells were assessed for three distinct effector functions , all mediated by Fc receptors .
	manualset3
90750	3	399088	13	NULL	NULL	0	NULL	control cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Human monocyte-derived macrophages treated with recombinant IFN-gamma ( rIFN-gamma ) and control cells were assessed for three distinct effector functions , all mediated by Fc receptors .
	manualset3
90751	4	399088	13	NULL	NULL	0	NULL	 effector functions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Human monocyte-derived macrophages treated with recombinant IFN-gamma ( rIFN-gamma ) and control cells were assessed for three distinct effector functions , all mediated by Fc receptors .
	manualset3
90752	5	399088	13	NULL	NULL	NULL	NULL	 Fc receptors	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human monocyte-derived macrophages treated with recombinant IFN-gamma ( rIFN-gamma ) and control cells were assessed for three distinct effector functions , all mediated by Fc receptors .
	manualset3
90755	1	399089	13	NULL	NULL	0	NULL	Human paleopathology 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Human paleopathology has the potential of enriching what we can reconstruct about the lives of our recent and ancient ancestors .
	manualset3
90761	2	399089	13	NULL	NULL	0	NULL	lives 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Human paleopathology has the potential of enriching what we can reconstruct about the lives of our recent and ancient ancestors .
	manualset3
90763	3	399089	13	NULL	NULL	NULL	NULL	recent ancestors	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human paleopathology has the potential of enriching what we can reconstruct about the lives of our recent and ancient ancestors .
	manualset3
91077	4	399089	13	NULL	NULL	0	NULL	ancient ancestors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Human paleopathology has the potential of enriching what we can reconstruct about the lives of our recent and ancient ancestors .
	manualset3
90766	1	399090	13	NULL	NULL	0	NULL	Human pancreatic kallikrein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human pancreatic kallikrein ( H. Panc .
	manualset3
90767	2	399090	13	NULL	NULL	0	NULL	H. Panc . 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Human pancreatic kallikrein ( H. Panc .
	manualset3
90768	1	399091	13	NULL	NULL	0	NULL	Human parvovirus B19 infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Human parvovirus B19 infection during pregnancy can result in fetal hydrops and death .
	manualset3
90769	2	399091	13	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Human parvovirus B19 infection during pregnancy can result in fetal hydrops and death .
	manualset3
90770	3	399091	13	NULL	NULL	NULL	NULL	 fetal hydrops	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human parvovirus B19 infection during pregnancy can result in fetal hydrops and death .
	manualset3
90771	4	399091	13	NULL	NULL	0	NULL	death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Human parvovirus B19 infection during pregnancy can result in fetal hydrops and death .
	manualset3
90772	1	399092	13	NULL	NULL	0	NULL	Human recombinant palmitoyl-protein thioesterase-1 ( PPT1 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human recombinant palmitoyl-protein thioesterase-1 ( PPT1 ) for preclinical evaluation of enzyme replacement therapy for infantile neuronal ceroid lipofuscinosis .
	manualset3
90773	2	399092	13	NULL	NULL	NULL	NULL	preclinical evaluation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human recombinant palmitoyl-protein thioesterase-1 ( PPT1 ) for preclinical evaluation of enzyme replacement therapy for infantile neuronal ceroid lipofuscinosis .
	manualset3
90774	3	399092	13	NULL	NULL	0	NULL	enzyme replacement therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Human recombinant palmitoyl-protein thioesterase-1 ( PPT1 ) for preclinical evaluation of enzyme replacement therapy for infantile neuronal ceroid lipofuscinosis .
	manualset3
90775	4	399092	13	NULL	NULL	NULL	NULL	 infantile neuronal ceroid lipofuscinosis 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human recombinant palmitoyl-protein thioesterase-1 ( PPT1 ) for preclinical evaluation of enzyme replacement therapy for infantile neuronal ceroid lipofuscinosis .
	manualset3
90776	1	399093	13	NULL	NULL	0	NULL	Human red blood cells ( H-RBC ) 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Human red blood cells ( H-RBC ) , sensitized by specific rabbit antihuman hemolysin , showed a significant increase in susceptibility to complement lysis after rigidification of the membrane lipid layer by incorporation of cholesterol ( p less than 0.001 ) .
	manualset3
90777	2	399093	13	NULL	NULL	0	NULL	rabbit antihuman hemolysin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human red blood cells ( H-RBC ) , sensitized by specific rabbit antihuman hemolysin , showed a significant increase in susceptibility to complement lysis after rigidification of the membrane lipid layer by incorporation of cholesterol ( p less than 0.001 ) .
	manualset3
90778	3	399093	13	NULL	NULL	0	NULL	 susceptibility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Human red blood cells ( H-RBC ) , sensitized by specific rabbit antihuman hemolysin , showed a significant increase in susceptibility to complement lysis after rigidification of the membrane lipid layer by incorporation of cholesterol ( p less than 0.001 ) .
	manualset3
90779	4	399093	13	NULL	NULL	0	NULL	complement lysis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Human red blood cells ( H-RBC ) , sensitized by specific rabbit antihuman hemolysin , showed a significant increase in susceptibility to complement lysis after rigidification of the membrane lipid layer by incorporation of cholesterol ( p less than 0.001 ) .
	manualset3
90780	5	399093	13	NULL	NULL	0	NULL	rigidification 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Human red blood cells ( H-RBC ) , sensitized by specific rabbit antihuman hemolysin , showed a significant increase in susceptibility to complement lysis after rigidification of the membrane lipid layer by incorporation of cholesterol ( p less than 0.001 ) .
	manualset3
90781	6	399093	13	NULL	NULL	0	NULL	membrane lipid layer 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Human red blood cells ( H-RBC ) , sensitized by specific rabbit antihuman hemolysin , showed a significant increase in susceptibility to complement lysis after rigidification of the membrane lipid layer by incorporation of cholesterol ( p less than 0.001 ) .
	manualset3
90782	7	399093	13	NULL	NULL	0	NULL	incorporation of cholesterol	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Human red blood cells ( H-RBC ) , sensitized by specific rabbit antihuman hemolysin , showed a significant increase in susceptibility to complement lysis after rigidification of the membrane lipid layer by incorporation of cholesterol ( p less than 0.001 ) .
	manualset3
90783	8	399093	13	NULL	NULL	0	NULL	p less than 0.001 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Human red blood cells ( H-RBC ) , sensitized by specific rabbit antihuman hemolysin , showed a significant increase in susceptibility to complement lysis after rigidification of the membrane lipid layer by incorporation of cholesterol ( p less than 0.001 ) .
	manualset3
90784	1	399094	13	NULL	NULL	0	NULL	Human ribonucleotide reductase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human ribonucleotide reductase was less sensitive to the inhibitory effects of A1110U and its iron-complex .
	manualset3
90785	2	399094	13	NULL	NULL	NULL	NULL	inhibitory effects	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human ribonucleotide reductase was less sensitive to the inhibitory effects of A1110U and its iron-complex .
	manualset3
90786	3	399094	13	NULL	NULL	0	NULL	 A1110U	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Human ribonucleotide reductase was less sensitive to the inhibitory effects of A1110U and its iron-complex .
	manualset3
90787	4	399094	13	NULL	NULL	0	NULL	iron-complex	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Human ribonucleotide reductase was less sensitive to the inhibitory effects of A1110U and its iron-complex .
	manualset3
90788	1	399095	13	NULL	NULL	0	NULL	Human ribosomal protein L7	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human ribosomal protein L7 incorporates an ER-binding characteristic .
	manualset3
90789	2	399095	13	NULL	NULL	0	NULL	ER-binding characteristic	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Human ribosomal protein L7 incorporates an ER-binding characteristic .
	manualset3
90790	1	399096	13	NULL	NULL	0	NULL	 promotion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( The promotion of plant growth by ultraviolet radiation ) .
	manualset3
90791	2	399096	13	NULL	NULL	0	NULL	plant growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( The promotion of plant growth by ultraviolet radiation ) .
	manualset3
90792	3	399096	13	NULL	NULL	0	NULL	 ultraviolet radiation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	( The promotion of plant growth by ultraviolet radiation ) .
	manualset3
90793	1	399097	13	NULL	NULL	0	NULL	Human serum holo-transferrin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human serum holo-transferrin was labeled with 99mTc using pre-reduction with 2-mercaptoethanol .
	manualset3
90794	2	399097	13	NULL	NULL	0	NULL	99mTc	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Human serum holo-transferrin was labeled with 99mTc using pre-reduction with 2-mercaptoethanol .
	manualset3
90795	3	399097	13	NULL	NULL	0	NULL	 pre-reduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Human serum holo-transferrin was labeled with 99mTc using pre-reduction with 2-mercaptoethanol .
	manualset3
90796	4	399097	13	NULL	NULL	0	NULL	2-mercaptoethanol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Human serum holo-transferrin was labeled with 99mTc using pre-reduction with 2-mercaptoethanol .
	manualset3
90797	1	399098	13	NULL	NULL	0	NULL	Human splenic marginal zone B cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Human splenic marginal zone B cells lack expression of activation-induced cytidine deaminase .
	manualset3
90798	2	399098	13	NULL	NULL	0	NULL	 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Human splenic marginal zone B cells lack expression of activation-induced cytidine deaminase .
	manualset3
90799	3	399098	13	NULL	NULL	0	NULL	activation-induced cytidine deaminase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human splenic marginal zone B cells lack expression of activation-induced cytidine deaminase .
	manualset3
90800	1	399099	13	NULL	NULL	0	NULL	Huntington 's disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Huntington 's disease : seeing the pathogenic process through a genetic lens .
	manualset3
90801	2	399099	13	NULL	NULL	0	NULL	pathogenic process	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Huntington 's disease : seeing the pathogenic process through a genetic lens .
	manualset3
90802	3	399099	13	NULL	NULL	NULL	NULL	 genetic lens	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Huntington 's disease : seeing the pathogenic process through a genetic lens .
	manualset3
90803	1	399100	13	NULL	NULL	0	NULL	Hyaluronic acid ( HA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyaluronic acid ( HA ) is a natural biopolymer with unique physiochemical and biological properties and finds a wide range of applications in biomedical and cosmetic fields .
	manualset3
90804	2	399100	13	NULL	NULL	NULL	NULL	natural biopolymer	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hyaluronic acid ( HA ) is a natural biopolymer with unique physiochemical and biological properties and finds a wide range of applications in biomedical and cosmetic fields .
	manualset3
90805	3	399100	13	NULL	NULL	0	NULL	applications	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyaluronic acid ( HA ) is a natural biopolymer with unique physiochemical and biological properties and finds a wide range of applications in biomedical and cosmetic fields .
	manualset3
90806	4	399100	13	NULL	NULL	0	NULL	biomedical fields	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyaluronic acid ( HA ) is a natural biopolymer with unique physiochemical and biological properties and finds a wide range of applications in biomedical and cosmetic fields .
	manualset3
90807	5	399100	13	NULL	NULL	0	NULL	cosmetic fields	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyaluronic acid ( HA ) is a natural biopolymer with unique physiochemical and biological properties and finds a wide range of applications in biomedical and cosmetic fields .
	manualset3
90808	1	399101	13	NULL	NULL	0	NULL	Hyaluronic acid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyaluronic acid and glycerol are viable carriers for demineralized bone matrices .
	manualset3
90809	2	399101	13	NULL	NULL	0	NULL	glycerol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyaluronic acid and glycerol are viable carriers for demineralized bone matrices .
	manualset3
90810	3	399101	13	NULL	NULL	0	NULL	carriers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyaluronic acid and glycerol are viable carriers for demineralized bone matrices .
	manualset3
90811	4	399101	13	NULL	NULL	NULL	NULL	demineralized bone matrices	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hyaluronic acid and glycerol are viable carriers for demineralized bone matrices .
	manualset3
90812	1	399102	13	NULL	NULL	NULL	NULL	Hybrid poplar response	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hybrid poplar and forest soil response to municipal and industrial by-products : a greenhouse study .
	manualset3
90813	2	399102	13	NULL	NULL	0	NULL	forest soil response	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Hybrid poplar and forest soil response to municipal and industrial by-products : a greenhouse study .
	manualset3
90814	3	399102	13	NULL	NULL	0	NULL	municipal by-products	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hybrid poplar and forest soil response to municipal and industrial by-products : a greenhouse study .
	manualset3
90815	4	399102	13	NULL	NULL	0	NULL	industrial by-products	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hybrid poplar and forest soil response to municipal and industrial by-products : a greenhouse study .
	manualset3
90816	5	399102	13	NULL	NULL	0	NULL	greenhouse study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hybrid poplar and forest soil response to municipal and industrial by-products : a greenhouse study .
	manualset3
90817	1	399103	13	NULL	NULL	0	NULL	Anatomical studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Anatomical studies on the structure of joints of the foot in south Kyushu Japanese .
	manualset3
90818	2	399103	13	NULL	NULL	0	NULL	structure of joints of the foot 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Anatomical studies on the structure of joints of the foot in south Kyushu Japanese .
	manualset3
90819	3	399103	13	NULL	NULL	0	NULL	south Kyushu Japanese	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Anatomical studies on the structure of joints of the foot in south Kyushu Japanese .
	manualset3
90820	1	399104	13	NULL	NULL	0	NULL	Hybridization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hybridization both on Southern blots and in situ as well as sequence analysis show that this subset is most closely related , as expected , to sequences on HSA 17 .
	manualset3
90821	2	399104	13	NULL	NULL	0	NULL	 Southern blots	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hybridization both on Southern blots and in situ as well as sequence analysis show that this subset is most closely related , as expected , to sequences on HSA 17 .
	manualset3
90822	3	399104	13	NULL	NULL	0	NULL	sequence analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hybridization both on Southern blots and in situ as well as sequence analysis show that this subset is most closely related , as expected , to sequences on HSA 17 .
	manualset3
90823	4	399104	13	NULL	NULL	0	NULL	subset	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Hybridization both on Southern blots and in situ as well as sequence analysis show that this subset is most closely related , as expected , to sequences on HSA 17 .
	manualset3
90824	5	399104	13	NULL	NULL	0	NULL	sequences on HSA 17	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Hybridization both on Southern blots and in situ as well as sequence analysis show that this subset is most closely related , as expected , to sequences on HSA 17 .
	manualset3
90825	1	399105	13	NULL	NULL	0	NULL	Hydration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydration and ionization of CO2 is facilitated by elevated hydrostatic pressure because a negative volume change ( delta V & lt ; 0 ) accompanies the chemical reaction .
	manualset3
90826	2	399105	13	NULL	NULL	0	NULL	 ionization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydration and ionization of CO2 is facilitated by elevated hydrostatic pressure because a negative volume change ( delta V & lt ; 0 ) accompanies the chemical reaction .
	manualset3
90827	3	399105	13	NULL	NULL	0	NULL	CO2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydration and ionization of CO2 is facilitated by elevated hydrostatic pressure because a negative volume change ( delta V & lt ; 0 ) accompanies the chemical reaction .
	manualset3
90828	4	399105	13	NULL	NULL	NULL	NULL	hydrostatic pressure	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hydration and ionization of CO2 is facilitated by elevated hydrostatic pressure because a negative volume change ( delta V & lt ; 0 ) accompanies the chemical reaction .
	manualset3
90829	5	399105	13	NULL	NULL	NULL	NULL	negative volume change 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hydration and ionization of CO2 is facilitated by elevated hydrostatic pressure because a negative volume change ( delta V & lt ; 0 ) accompanies the chemical reaction .
	manualset3
90830	6	399105	13	NULL	NULL	0	NULL	delta V & lt ; 0	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydration and ionization of CO2 is facilitated by elevated hydrostatic pressure because a negative volume change ( delta V & lt ; 0 ) accompanies the chemical reaction .
	manualset3
90831	7	399105	13	NULL	NULL	0	NULL	chemical reaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydration and ionization of CO2 is facilitated by elevated hydrostatic pressure because a negative volume change ( delta V & lt ; 0 ) accompanies the chemical reaction .
	manualset3
90832	1	399106	13	NULL	NULL	NULL	NULL	Hydrodynamic calculations	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hydrodynamic calculations lead to the conclusion that chymotryptic ( or ethylenediaminetetraacetic acid ) myosin S1 in solution ( hydrated ) , at 1-5 degrees C , can be modeled as a prolate ellipsoid , with an axial ratio lying between p = 1.0 and 2.5 ( major axis between 100.5 A , for p = 1.0 , and 162.5 A , for p = 2.5 ) .
	manualset3
90833	2	399106	13	NULL	NULL	0	NULL	conclusion	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrodynamic calculations lead to the conclusion that chymotryptic ( or ethylenediaminetetraacetic acid ) myosin S1 in solution ( hydrated ) , at 1-5 degrees C , can be modeled as a prolate ellipsoid , with an axial ratio lying between p = 1.0 and 2.5 ( major axis between 100.5 A , for p = 1.0 , and 162.5 A , for p = 2.5 ) .
	manualset3
90834	3	399106	13	NULL	NULL	0	NULL	ethylenediaminetetraacetic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrodynamic calculations lead to the conclusion that chymotryptic ( or ethylenediaminetetraacetic acid ) myosin S1 in solution ( hydrated ) , at 1-5 degrees C , can be modeled as a prolate ellipsoid , with an axial ratio lying between p = 1.0 and 2.5 ( major axis between 100.5 A , for p = 1.0 , and 162.5 A , for p = 2.5 ) .
	manualset3
90835	4	399106	13	NULL	NULL	NULL	NULL	chymotryptic myosin S1 in solution	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hydrodynamic calculations lead to the conclusion that chymotryptic ( or ethylenediaminetetraacetic acid ) myosin S1 in solution ( hydrated ) , at 1-5 degrees C , can be modeled as a prolate ellipsoid , with an axial ratio lying between p = 1.0 and 2.5 ( major axis between 100.5 A , for p = 1.0 , and 162.5 A , for p = 2.5 ) .
	manualset3
90837	6	399106	13	NULL	NULL	0	NULL	1-5 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrodynamic calculations lead to the conclusion that chymotryptic ( or ethylenediaminetetraacetic acid ) myosin S1 in solution ( hydrated ) , at 1-5 degrees C , can be modeled as a prolate ellipsoid , with an axial ratio lying between p = 1.0 and 2.5 ( major axis between 100.5 A , for p = 1.0 , and 162.5 A , for p = 2.5 ) .
	manualset3
90838	7	399106	13	NULL	NULL	NULL	NULL	prolate ellipsoid	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hydrodynamic calculations lead to the conclusion that chymotryptic ( or ethylenediaminetetraacetic acid ) myosin S1 in solution ( hydrated ) , at 1-5 degrees C , can be modeled as a prolate ellipsoid , with an axial ratio lying between p = 1.0 and 2.5 ( major axis between 100.5 A , for p = 1.0 , and 162.5 A , for p = 2.5 ) .
	manualset3
90839	8	399106	13	NULL	NULL	0	NULL	axial ratio	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrodynamic calculations lead to the conclusion that chymotryptic ( or ethylenediaminetetraacetic acid ) myosin S1 in solution ( hydrated ) , at 1-5 degrees C , can be modeled as a prolate ellipsoid , with an axial ratio lying between p = 1.0 and 2.5 ( major axis between 100.5 A , for p = 1.0 , and 162.5 A , for p = 2.5 ) .
	manualset3
90840	9	399106	13	NULL	NULL	0	NULL	between p = 1.0 and 2.5 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrodynamic calculations lead to the conclusion that chymotryptic ( or ethylenediaminetetraacetic acid ) myosin S1 in solution ( hydrated ) , at 1-5 degrees C , can be modeled as a prolate ellipsoid , with an axial ratio lying between p = 1.0 and 2.5 ( major axis between 100.5 A , for p = 1.0 , and 162.5 A , for p = 2.5 ) .
	manualset3
90841	10	399106	13	NULL	NULL	NULL	NULL	major axis	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hydrodynamic calculations lead to the conclusion that chymotryptic ( or ethylenediaminetetraacetic acid ) myosin S1 in solution ( hydrated ) , at 1-5 degrees C , can be modeled as a prolate ellipsoid , with an axial ratio lying between p = 1.0 and 2.5 ( major axis between 100.5 A , for p = 1.0 , and 162.5 A , for p = 2.5 ) .
	manualset3
90842	11	399106	13	NULL	NULL	0	NULL	100.5 A , for p = 1.0	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrodynamic calculations lead to the conclusion that chymotryptic ( or ethylenediaminetetraacetic acid ) myosin S1 in solution ( hydrated ) , at 1-5 degrees C , can be modeled as a prolate ellipsoid , with an axial ratio lying between p = 1.0 and 2.5 ( major axis between 100.5 A , for p = 1.0 , and 162.5 A , for p = 2.5 ) .
	manualset3
90843	12	399106	13	NULL	NULL	0	NULL	162.5 A , for p = 2.5	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrodynamic calculations lead to the conclusion that chymotryptic ( or ethylenediaminetetraacetic acid ) myosin S1 in solution ( hydrated ) , at 1-5 degrees C , can be modeled as a prolate ellipsoid , with an axial ratio lying between p = 1.0 and 2.5 ( major axis between 100.5 A , for p = 1.0 , and 162.5 A , for p = 2.5 ) .
	manualset3
90844	1	399107	13	NULL	NULL	0	NULL	Hydrogels 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogels have been synthesized starting from water solutions of carboxymethylcellulose sodium salt and hydroxyethylcellulose , chemically crosslinked with divinylsulphone .
	manualset3
90845	2	399107	13	NULL	NULL	0	NULL	water solutions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogels have been synthesized starting from water solutions of carboxymethylcellulose sodium salt and hydroxyethylcellulose , chemically crosslinked with divinylsulphone .
	manualset3
90846	3	399107	13	NULL	NULL	0	NULL	carboxymethylcellulose sodium salt	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogels have been synthesized starting from water solutions of carboxymethylcellulose sodium salt and hydroxyethylcellulose , chemically crosslinked with divinylsulphone .
	manualset3
90847	4	399107	13	NULL	NULL	0	NULL	hydroxyethylcellulose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogels have been synthesized starting from water solutions of carboxymethylcellulose sodium salt and hydroxyethylcellulose , chemically crosslinked with divinylsulphone .
	manualset3
90848	5	399107	13	NULL	NULL	0	NULL	divinylsulphone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogels have been synthesized starting from water solutions of carboxymethylcellulose sodium salt and hydroxyethylcellulose , chemically crosslinked with divinylsulphone .
	manualset3
90849	1	399108	13	NULL	NULL	0	NULL	Hydrogen-deuterium exchange experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogen-deuterium exchange experiments were performed to map with higher resolution the conformational changes induced by metal binding .
	manualset3
90851	3	399108	13	NULL	NULL	NULL	NULL	higher resolution	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hydrogen-deuterium exchange experiments were performed to map with higher resolution the conformational changes induced by metal binding .
	manualset3
90852	4	399108	13	NULL	NULL	0	NULL	conformational changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogen-deuterium exchange experiments were performed to map with higher resolution the conformational changes induced by metal binding .
	manualset3
90853	5	399108	13	NULL	NULL	0	NULL	metal binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogen-deuterium exchange experiments were performed to map with higher resolution the conformational changes induced by metal binding .
	manualset3
90854	1	399109	13	NULL	NULL	0	NULL	Hydrogen-isotopic compositions 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogen-isotopic compositions of carbonate and maskelynite in Allan Hills ( ALH ) 84001 were measured by secondary ion mass spectrometry ( SIMS ) .
	manualset3
90855	2	399109	13	NULL	NULL	0	NULL	carbonate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogen-isotopic compositions of carbonate and maskelynite in Allan Hills ( ALH ) 84001 were measured by secondary ion mass spectrometry ( SIMS ) .
	manualset3
90856	3	399109	13	NULL	NULL	0	NULL	maskelynite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogen-isotopic compositions of carbonate and maskelynite in Allan Hills ( ALH ) 84001 were measured by secondary ion mass spectrometry ( SIMS ) .
	manualset3
90857	4	399109	13	NULL	NULL	0	NULL	Allan Hills ( ALH ) 84001	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogen-isotopic compositions of carbonate and maskelynite in Allan Hills ( ALH ) 84001 were measured by secondary ion mass spectrometry ( SIMS ) .
	manualset3
90858	5	399109	13	NULL	NULL	0	NULL	secondary ion mass spectrometry ( SIMS )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogen-isotopic compositions of carbonate and maskelynite in Allan Hills ( ALH ) 84001 were measured by secondary ion mass spectrometry ( SIMS ) .
	manualset3
90859	1	399110	13	NULL	NULL	0	NULL	reaction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( The reaction of the circulation following intravenous application of bradykinin in man ) .
	manualset3
90860	2	399110	13	NULL	NULL	0	NULL	circulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( The reaction of the circulation following intravenous application of bradykinin in man ) .
	manualset3
90861	3	399110	13	NULL	NULL	0	NULL	intravenous application	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( The reaction of the circulation following intravenous application of bradykinin in man ) .
	manualset3
90862	4	399110	13	NULL	NULL	0	NULL	bradykinin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( The reaction of the circulation following intravenous application of bradykinin in man ) .
	manualset3
90863	5	399110	13	NULL	NULL	NULL	NULL	man	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The reaction of the circulation following intravenous application of bradykinin in man ) .
	manualset3
90864	1	399111	13	NULL	NULL	0	NULL	Hydrogen bonding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogen bonding in water clusters and their ionized counterparts .
	manualset3
90865	2	399111	13	NULL	NULL	0	NULL	water clusters	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogen bonding in water clusters and their ionized counterparts .
	manualset3
90866	3	399111	13	NULL	NULL	0	NULL	ionized counterparts	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogen bonding in water clusters and their ionized counterparts .
	manualset3
90867	1	399112	13	NULL	NULL	0	NULL	Hydrogen bonds	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogen bonds between water molecules and carboxylate O atoms link neighbouring ( 4 , 4 ) networks , yielding a three-dimensional alpha-polonium net .
	manualset3
90868	2	399112	13	NULL	NULL	0	NULL	water molecules 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogen bonds between water molecules and carboxylate O atoms link neighbouring ( 4 , 4 ) networks , yielding a three-dimensional alpha-polonium net .
	manualset3
90869	3	399112	13	NULL	NULL	0	NULL	carboxylate O atoms	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogen bonds between water molecules and carboxylate O atoms link neighbouring ( 4 , 4 ) networks , yielding a three-dimensional alpha-polonium net .
	manualset3
90872	6	399112	13	NULL	NULL	0	NULL	three-dimensional alpha-polonium net	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogen bonds between water molecules and carboxylate O atoms link neighbouring ( 4 , 4 ) networks , yielding a three-dimensional alpha-polonium net .
	manualset3
92370	4	399112	13	NULL	NULL	0	NULL	neighbouring ( 4 , 4 ) networks	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogen bonds between water molecules and carboxylate O atoms link neighbouring ( 4 , 4 ) networks , yielding a three-dimensional alpha-polonium net .
	manualset3
90871	1	399113	13	NULL	NULL	NULL	NULL	Hydrogen peroxide	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hydrogen peroxide stimulated bone resorption in a concentration-dependent manner in calvarial organ cultures with a maximal effect at 1 mumol/L ( 45Ca release ; treated/control = 1.6 + / - 0.07 ; p & lt ; 0.001 from control ) .
	manualset3
90873	2	399113	13	NULL	NULL	0	NULL	bone resorption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogen peroxide stimulated bone resorption in a concentration-dependent manner in calvarial organ cultures with a maximal effect at 1 mumol/L ( 45Ca release ; treated/control = 1.6 + / - 0.07 ; p & lt ; 0.001 from control ) .
	manualset3
90874	3	399113	13	NULL	NULL	0	NULL	concentration-dependent manner	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogen peroxide stimulated bone resorption in a concentration-dependent manner in calvarial organ cultures with a maximal effect at 1 mumol/L ( 45Ca release ; treated/control = 1.6 + / - 0.07 ; p & lt ; 0.001 from control ) .
	manualset3
90875	4	399113	13	NULL	NULL	0	NULL	calvarial organ cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogen peroxide stimulated bone resorption in a concentration-dependent manner in calvarial organ cultures with a maximal effect at 1 mumol/L ( 45Ca release ; treated/control = 1.6 + / - 0.07 ; p & lt ; 0.001 from control ) .
	manualset3
90876	5	399113	13	NULL	NULL	0	NULL	effect at 1 mumol/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogen peroxide stimulated bone resorption in a concentration-dependent manner in calvarial organ cultures with a maximal effect at 1 mumol/L ( 45Ca release ; treated/control = 1.6 + / - 0.07 ; p & lt ; 0.001 from control ) .
	manualset3
90877	6	399113	13	NULL	NULL	0	NULL	45Ca release	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogen peroxide stimulated bone resorption in a concentration-dependent manner in calvarial organ cultures with a maximal effect at 1 mumol/L ( 45Ca release ; treated/control = 1.6 + / - 0.07 ; p & lt ; 0.001 from control ) .
	manualset3
90878	7	399113	13	NULL	NULL	0	NULL	treated/control = 1.6 + / - 0.07 ; p & lt ; 0.001 from control	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogen peroxide stimulated bone resorption in a concentration-dependent manner in calvarial organ cultures with a maximal effect at 1 mumol/L ( 45Ca release ; treated/control = 1.6 + / - 0.07 ; p & lt ; 0.001 from control ) .
	manualset3
90879	1	399114	13	NULL	NULL	0	NULL	Hydrogen sulfide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogen sulfide : its production and functions .
	manualset3
90880	2	399114	13	NULL	NULL	0	NULL	production 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogen sulfide : its production and functions .
	manualset3
90881	3	399114	13	NULL	NULL	0	NULL	functions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogen sulfide : its production and functions .
	manualset3
90882	1	399115	13	NULL	NULL	NULL	NULL	Hydrogen transfer reaction	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hydrogen transfer reaction on the surface of an oxide catalyst .
	manualset3
90883	2	399115	13	NULL	NULL	0	NULL	surface of an oxide catalyst	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrogen transfer reaction on the surface of an oxide catalyst .
	manualset3
90884	1	399116	13	NULL	NULL	NULL	NULL	Hydrolysis	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hydrolysis of trehalose in yeast depends on neutral trehalase and acid trehalase ( Ath1 ) .
	manualset3
90885	2	399116	13	NULL	NULL	NULL	NULL	trehalose	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hydrolysis of trehalose in yeast depends on neutral trehalase and acid trehalase ( Ath1 ) .
	manualset3
90886	3	399116	13	NULL	NULL	0	NULL	yeast	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrolysis of trehalose in yeast depends on neutral trehalase and acid trehalase ( Ath1 ) .
	manualset3
90887	4	399116	13	NULL	NULL	NULL	NULL	neutral trehalase	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hydrolysis of trehalose in yeast depends on neutral trehalase and acid trehalase ( Ath1 ) .
	manualset3
90888	5	399116	13	NULL	NULL	NULL	NULL	acid trehalase ( Ath1 )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hydrolysis of trehalose in yeast depends on neutral trehalase and acid trehalase ( Ath1 ) .
	manualset3
90889	1	399117	13	NULL	NULL	0	NULL	Hydrolytic kinetics	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrolytic kinetics of lithospermic acid B extracted from roots of Salvia miltiorrhiza .
	manualset3
90890	2	399117	13	NULL	NULL	0	NULL	lithospermic acid B	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrolytic kinetics of lithospermic acid B extracted from roots of Salvia miltiorrhiza .
	manualset3
90891	3	399117	13	NULL	NULL	0	NULL	 roots	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrolytic kinetics of lithospermic acid B extracted from roots of Salvia miltiorrhiza .
	manualset3
90892	4	399117	13	NULL	NULL	0	NULL	Salvia miltiorrhiza	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrolytic kinetics of lithospermic acid B extracted from roots of Salvia miltiorrhiza .
	manualset3
90893	1	399118	13	NULL	NULL	0	NULL	Hydrotalcite-like catalysts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrotalcite-like catalysts were synthesized by coprecipitation and modified co-precipitation by the impregnation method and those were promoted by the addition of noble metals .
	manualset3
90894	2	399118	13	NULL	NULL	0	NULL	coprecipitation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrotalcite-like catalysts were synthesized by coprecipitation and modified co-precipitation by the impregnation method and those were promoted by the addition of noble metals .
	manualset3
90895	3	399118	13	NULL	NULL	0	NULL	co-precipitation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrotalcite-like catalysts were synthesized by coprecipitation and modified co-precipitation by the impregnation method and those were promoted by the addition of noble metals .
	manualset3
90896	4	399118	13	NULL	NULL	0	NULL	 impregnation method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrotalcite-like catalysts were synthesized by coprecipitation and modified co-precipitation by the impregnation method and those were promoted by the addition of noble metals .
	manualset3
90897	5	399118	13	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydrotalcite-like catalysts were synthesized by coprecipitation and modified co-precipitation by the impregnation method and those were promoted by the addition of noble metals .
	manualset3
90898	6	399118	13	NULL	NULL	NULL	NULL	noble metals 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hydrotalcite-like catalysts were synthesized by coprecipitation and modified co-precipitation by the impregnation method and those were promoted by the addition of noble metals .
	manualset3
90899	1	399119	13	NULL	NULL	0	NULL	Hydroxy-naphthoquinones	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydroxy-naphthoquinones are competitive inhibitors of the cytochrome bc ( 1 ) complex that bind to the ubiquinol oxidation site between cytochrome b and the iron-sulfur protein and presumably mimic a transition state in the ubiquinol oxidation reaction catalyzed by the enzyme .
	manualset3
90900	2	399119	13	NULL	NULL	NULL	NULL	competitive inhibitors	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hydroxy-naphthoquinones are competitive inhibitors of the cytochrome bc ( 1 ) complex that bind to the ubiquinol oxidation site between cytochrome b and the iron-sulfur protein and presumably mimic a transition state in the ubiquinol oxidation reaction catalyzed by the enzyme .
	manualset3
90901	3	399119	13	NULL	NULL	0	NULL	cytochrome bc ( 1 ) complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydroxy-naphthoquinones are competitive inhibitors of the cytochrome bc ( 1 ) complex that bind to the ubiquinol oxidation site between cytochrome b and the iron-sulfur protein and presumably mimic a transition state in the ubiquinol oxidation reaction catalyzed by the enzyme .
	manualset3
90902	4	399119	13	NULL	NULL	0	NULL	bind	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydroxy-naphthoquinones are competitive inhibitors of the cytochrome bc ( 1 ) complex that bind to the ubiquinol oxidation site between cytochrome b and the iron-sulfur protein and presumably mimic a transition state in the ubiquinol oxidation reaction catalyzed by the enzyme .
	manualset3
90903	5	399119	13	NULL	NULL	0	NULL	 ubiquinol oxidation site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydroxy-naphthoquinones are competitive inhibitors of the cytochrome bc ( 1 ) complex that bind to the ubiquinol oxidation site between cytochrome b and the iron-sulfur protein and presumably mimic a transition state in the ubiquinol oxidation reaction catalyzed by the enzyme .
	manualset3
90904	6	399119	13	NULL	NULL	0	NULL	cytochrome b	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydroxy-naphthoquinones are competitive inhibitors of the cytochrome bc ( 1 ) complex that bind to the ubiquinol oxidation site between cytochrome b and the iron-sulfur protein and presumably mimic a transition state in the ubiquinol oxidation reaction catalyzed by the enzyme .
	manualset3
90905	7	399119	13	NULL	NULL	0	NULL	iron-sulfur protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydroxy-naphthoquinones are competitive inhibitors of the cytochrome bc ( 1 ) complex that bind to the ubiquinol oxidation site between cytochrome b and the iron-sulfur protein and presumably mimic a transition state in the ubiquinol oxidation reaction catalyzed by the enzyme .
	manualset3
90906	8	399119	13	NULL	NULL	0	NULL	transition state	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydroxy-naphthoquinones are competitive inhibitors of the cytochrome bc ( 1 ) complex that bind to the ubiquinol oxidation site between cytochrome b and the iron-sulfur protein and presumably mimic a transition state in the ubiquinol oxidation reaction catalyzed by the enzyme .
	manualset3
90907	9	399119	13	NULL	NULL	0	NULL	ubiquinol oxidation reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydroxy-naphthoquinones are competitive inhibitors of the cytochrome bc ( 1 ) complex that bind to the ubiquinol oxidation site between cytochrome b and the iron-sulfur protein and presumably mimic a transition state in the ubiquinol oxidation reaction catalyzed by the enzyme .
	manualset3
90908	10	399119	13	NULL	NULL	0	NULL	 enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydroxy-naphthoquinones are competitive inhibitors of the cytochrome bc ( 1 ) complex that bind to the ubiquinol oxidation site between cytochrome b and the iron-sulfur protein and presumably mimic a transition state in the ubiquinol oxidation reaction catalyzed by the enzyme .
	manualset3
90909	1	399120	13	NULL	NULL	0	NULL	Hydroxyl derivative 7b	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydroxyl derivative 7b showed the highest reactivity toward thiols and showed the strongest cytotoxicity in Hela S3 cells among the three derivatives having a different protecting group at the tert-hydroxyl group .
	manualset3
90910	2	399120	13	NULL	NULL	0	NULL	reactivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydroxyl derivative 7b showed the highest reactivity toward thiols and showed the strongest cytotoxicity in Hela S3 cells among the three derivatives having a different protecting group at the tert-hydroxyl group .
	manualset3
90911	3	399120	13	NULL	NULL	0	NULL	thiols 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydroxyl derivative 7b showed the highest reactivity toward thiols and showed the strongest cytotoxicity in Hela S3 cells among the three derivatives having a different protecting group at the tert-hydroxyl group .
	manualset3
90912	4	399120	13	NULL	NULL	0	NULL	cytotoxicity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydroxyl derivative 7b showed the highest reactivity toward thiols and showed the strongest cytotoxicity in Hela S3 cells among the three derivatives having a different protecting group at the tert-hydroxyl group .
	manualset3
90913	5	399120	13	NULL	NULL	0	NULL	Hela S3 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydroxyl derivative 7b showed the highest reactivity toward thiols and showed the strongest cytotoxicity in Hela S3 cells among the three derivatives having a different protecting group at the tert-hydroxyl group .
	manualset3
90914	6	399120	13	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydroxyl derivative 7b showed the highest reactivity toward thiols and showed the strongest cytotoxicity in Hela S3 cells among the three derivatives having a different protecting group at the tert-hydroxyl group .
	manualset3
90915	7	399120	13	NULL	NULL	0	NULL	derivatives 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydroxyl derivative 7b showed the highest reactivity toward thiols and showed the strongest cytotoxicity in Hela S3 cells among the three derivatives having a different protecting group at the tert-hydroxyl group .
	manualset3
90916	8	399120	13	NULL	NULL	NULL	NULL	protecting group 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hydroxyl derivative 7b showed the highest reactivity toward thiols and showed the strongest cytotoxicity in Hela S3 cells among the three derivatives having a different protecting group at the tert-hydroxyl group .
	manualset3
90917	9	399120	13	NULL	NULL	0	NULL	tert-hydroxyl group 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hydroxyl derivative 7b showed the highest reactivity toward thiols and showed the strongest cytotoxicity in Hela S3 cells among the three derivatives having a different protecting group at the tert-hydroxyl group .
	manualset3
90918	1	399121	13	NULL	NULL	NULL	NULL	Hyper-Raman scattering	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hyper-Raman scattering enhanced by anisotropic dimer plasmons on artificial nanostructures .
	manualset3
90920	3	399121	13	NULL	NULL	NULL	NULL	artificial nanostructures 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hyper-Raman scattering enhanced by anisotropic dimer plasmons on artificial nanostructures .
	manualset3
91078	4	399121	13	NULL	NULL	0	NULL	 anisotropic dimer plasmons	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyper-Raman scattering enhanced by anisotropic dimer plasmons on artificial nanostructures .
	manualset3
90919	1	399122	13	NULL	NULL	NULL	NULL	Hyperandrogenemia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hyperandrogenemia and hyperinsulinemia are conditions whose significance in terms of increasing both endometrial and breast cancer risks is increasingly recognized .
	manualset3
90921	2	399122	13	NULL	NULL	0	NULL	hyperinsulinemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperandrogenemia and hyperinsulinemia are conditions whose significance in terms of increasing both endometrial and breast cancer risks is increasingly recognized .
	manualset3
90922	3	399122	13	NULL	NULL	0	NULL	conditions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperandrogenemia and hyperinsulinemia are conditions whose significance in terms of increasing both endometrial and breast cancer risks is increasingly recognized .
	manualset3
90923	4	399122	13	NULL	NULL	0	NULL	significance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperandrogenemia and hyperinsulinemia are conditions whose significance in terms of increasing both endometrial and breast cancer risks is increasingly recognized .
	manualset3
90924	5	399122	13	NULL	NULL	0	NULL	endometrial cancer risks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperandrogenemia and hyperinsulinemia are conditions whose significance in terms of increasing both endometrial and breast cancer risks is increasingly recognized .
	manualset3
90925	6	399122	13	NULL	NULL	0	NULL	breast cancer risks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperandrogenemia and hyperinsulinemia are conditions whose significance in terms of increasing both endometrial and breast cancer risks is increasingly recognized .
	manualset3
90926	1	399123	13	NULL	NULL	0	NULL	Hypercalcemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypercalcemia , on the other hand , can be associated with increased extraosseous calcium and phosphate deposition leading to vascular calcification with an attendant mortality and morbidity .
	manualset3
90927	2	399123	13	NULL	NULL	NULL	NULL	extraosseous calcium	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hypercalcemia , on the other hand , can be associated with increased extraosseous calcium and phosphate deposition leading to vascular calcification with an attendant mortality and morbidity .
	manualset3
90928	3	399123	13	NULL	NULL	NULL	NULL	phosphate deposition	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hypercalcemia , on the other hand , can be associated with increased extraosseous calcium and phosphate deposition leading to vascular calcification with an attendant mortality and morbidity .
	manualset3
90929	4	399123	13	NULL	NULL	0	NULL	vascular calcification	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypercalcemia , on the other hand , can be associated with increased extraosseous calcium and phosphate deposition leading to vascular calcification with an attendant mortality and morbidity .
	manualset3
90930	5	399123	13	NULL	NULL	0	NULL	attendant	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypercalcemia , on the other hand , can be associated with increased extraosseous calcium and phosphate deposition leading to vascular calcification with an attendant mortality and morbidity .
	manualset3
90931	6	399123	13	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypercalcemia , on the other hand , can be associated with increased extraosseous calcium and phosphate deposition leading to vascular calcification with an attendant mortality and morbidity .
	manualset3
90932	7	399123	13	NULL	NULL	0	NULL	morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypercalcemia , on the other hand , can be associated with increased extraosseous calcium and phosphate deposition leading to vascular calcification with an attendant mortality and morbidity .
	manualset3
90933	1	399124	13	NULL	NULL	0	NULL	Hyperfractionated radiotherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperfractionated radiotherapy followed by adjuvant chemotherapy for nasopharyngeal cancer : report of seven cases .
	manualset3
90934	2	399124	13	NULL	NULL	0	NULL	adjuvant chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperfractionated radiotherapy followed by adjuvant chemotherapy for nasopharyngeal cancer : report of seven cases .
	manualset3
90935	3	399124	13	NULL	NULL	0	NULL	nasopharyngeal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperfractionated radiotherapy followed by adjuvant chemotherapy for nasopharyngeal cancer : report of seven cases .
	manualset3
90936	4	399124	13	NULL	NULL	0	NULL	report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperfractionated radiotherapy followed by adjuvant chemotherapy for nasopharyngeal cancer : report of seven cases .
	manualset3
90937	5	399124	13	NULL	NULL	0	NULL	seven	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperfractionated radiotherapy followed by adjuvant chemotherapy for nasopharyngeal cancer : report of seven cases .
	manualset3
90938	6	399124	13	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperfractionated radiotherapy followed by adjuvant chemotherapy for nasopharyngeal cancer : report of seven cases .
	manualset3
90939	1	399125	13	NULL	NULL	0	NULL	Hyperglycemia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperglycemia promotes the intracellular generation of superoxide anion and hydrogen peroxide , both of which have been linked to the activation of the mitochondrial apoptosis program .
	manualset3
90940	2	399125	13	NULL	NULL	0	NULL	intracellular generation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperglycemia promotes the intracellular generation of superoxide anion and hydrogen peroxide , both of which have been linked to the activation of the mitochondrial apoptosis program .
	manualset3
90941	3	399125	13	NULL	NULL	0	NULL	superoxide anion	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperglycemia promotes the intracellular generation of superoxide anion and hydrogen peroxide , both of which have been linked to the activation of the mitochondrial apoptosis program .
	manualset3
90942	4	399125	13	NULL	NULL	0	NULL	 hydrogen peroxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperglycemia promotes the intracellular generation of superoxide anion and hydrogen peroxide , both of which have been linked to the activation of the mitochondrial apoptosis program .
	manualset3
90944	6	399125	13	NULL	NULL	0	NULL	mitochondrial apoptosis program	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperglycemia promotes the intracellular generation of superoxide anion and hydrogen peroxide , both of which have been linked to the activation of the mitochondrial apoptosis program .
	manualset3
91079	7	399125	13	NULL	NULL	0	NULL	 activation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperglycemia promotes the intracellular generation of superoxide anion and hydrogen peroxide , both of which have been linked to the activation of the mitochondrial apoptosis program .
	manualset3
90943	1	399126	13	NULL	NULL	NULL	NULL	Hyperleptinemia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hyperleptinemia was associated with insulin resistance ( r = -0.57 ; P & lt ; 0.0001 ) and high waist to hip ratio ( r = 0.75 ; P & lt ; 0.0001 ) only in men .
	manualset3
90945	2	399126	13	NULL	NULL	0	NULL	insulin resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperleptinemia was associated with insulin resistance ( r = -0.57 ; P & lt ; 0.0001 ) and high waist to hip ratio ( r = 0.75 ; P & lt ; 0.0001 ) only in men .
	manualset3
90946	3	399126	13	NULL	NULL	0	NULL	 r = -0.57 ; P & lt ; 0.0001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperleptinemia was associated with insulin resistance ( r = -0.57 ; P & lt ; 0.0001 ) and high waist to hip ratio ( r = 0.75 ; P & lt ; 0.0001 ) only in men .
	manualset3
90947	4	399126	13	NULL	NULL	NULL	NULL	high waist to hip ratio ( r = 0.75 ; P & lt ; 0.0001 )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hyperleptinemia was associated with insulin resistance ( r = -0.57 ; P & lt ; 0.0001 ) and high waist to hip ratio ( r = 0.75 ; P & lt ; 0.0001 ) only in men .
	manualset3
90948	5	399126	13	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperleptinemia was associated with insulin resistance ( r = -0.57 ; P & lt ; 0.0001 ) and high waist to hip ratio ( r = 0.75 ; P & lt ; 0.0001 ) only in men .
	manualset3
90949	1	399127	13	NULL	NULL	0	NULL	Hyperosmolar non-ketotic diabetic coma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperosmolar non-ketotic diabetic coma following leptospirosis -- a case report .
	manualset3
90950	2	399127	13	NULL	NULL	0	NULL	leptospirosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperosmolar non-ketotic diabetic coma following leptospirosis -- a case report .
	manualset3
90951	3	399127	13	NULL	NULL	0	NULL	a case report 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperosmolar non-ketotic diabetic coma following leptospirosis -- a case report .
	manualset3
90952	1	399128	13	NULL	NULL	0	NULL	regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( The regulation of serum albumin in physiological and pathological conditions ( author 's transl ) ) .
	manualset3
90953	2	399128	13	NULL	NULL	0	NULL	serum albumin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( The regulation of serum albumin in physiological and pathological conditions ( author 's transl ) ) .
	manualset3
90954	3	399128	13	NULL	NULL	0	NULL	 physiological conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( The regulation of serum albumin in physiological and pathological conditions ( author 's transl ) ) .
	manualset3
90955	4	399128	13	NULL	NULL	0	NULL	pathological conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( The regulation of serum albumin in physiological and pathological conditions ( author 's transl ) ) .
	manualset3
90956	5	399128	13	NULL	NULL	0	NULL	author 's	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( The regulation of serum albumin in physiological and pathological conditions ( author 's transl ) ) .
	manualset3
90957	1	399129	13	NULL	NULL	0	NULL	Hyperphosphorylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperphosphorylation was dependent on L-voltage dependent Ca ( 2 + ) channels ( L-VDCC ) , N-methyl-d-aspartate ( NMDA ) and metabotropic glutamate receptors , as demonstrated by the specific inhibitors verapamil , DL-AP5 and MCPG , respectively .
	manualset3
90958	2	399129	13	NULL	NULL	0	NULL	L-voltage dependent Ca ( 2 + ) channels ( L-VDCC )	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperphosphorylation was dependent on L-voltage dependent Ca ( 2 + ) channels ( L-VDCC ) , N-methyl-d-aspartate ( NMDA ) and metabotropic glutamate receptors , as demonstrated by the specific inhibitors verapamil , DL-AP5 and MCPG , respectively .
	manualset3
90959	3	399129	13	NULL	NULL	0	NULL	N-methyl-d-aspartate ( NMDA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperphosphorylation was dependent on L-voltage dependent Ca ( 2 + ) channels ( L-VDCC ) , N-methyl-d-aspartate ( NMDA ) and metabotropic glutamate receptors , as demonstrated by the specific inhibitors verapamil , DL-AP5 and MCPG , respectively .
	manualset3
90960	4	399129	13	NULL	NULL	NULL	NULL	metabotropic glutamate receptors	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hyperphosphorylation was dependent on L-voltage dependent Ca ( 2 + ) channels ( L-VDCC ) , N-methyl-d-aspartate ( NMDA ) and metabotropic glutamate receptors , as demonstrated by the specific inhibitors verapamil , DL-AP5 and MCPG , respectively .
	manualset3
90961	5	399129	13	NULL	NULL	0	NULL	inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperphosphorylation was dependent on L-voltage dependent Ca ( 2 + ) channels ( L-VDCC ) , N-methyl-d-aspartate ( NMDA ) and metabotropic glutamate receptors , as demonstrated by the specific inhibitors verapamil , DL-AP5 and MCPG , respectively .
	manualset3
90962	6	399129	13	NULL	NULL	0	NULL	verapamil	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperphosphorylation was dependent on L-voltage dependent Ca ( 2 + ) channels ( L-VDCC ) , N-methyl-d-aspartate ( NMDA ) and metabotropic glutamate receptors , as demonstrated by the specific inhibitors verapamil , DL-AP5 and MCPG , respectively .
	manualset3
90963	7	399129	13	NULL	NULL	0	NULL	DL-AP5	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperphosphorylation was dependent on L-voltage dependent Ca ( 2 + ) channels ( L-VDCC ) , N-methyl-d-aspartate ( NMDA ) and metabotropic glutamate receptors , as demonstrated by the specific inhibitors verapamil , DL-AP5 and MCPG , respectively .
	manualset3
91080	8	399129	13	NULL	NULL	0	NULL	MCPG	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperphosphorylation was dependent on L-voltage dependent Ca ( 2 + ) channels ( L-VDCC ) , N-methyl-d-aspartate ( NMDA ) and metabotropic glutamate receptors , as demonstrated by the specific inhibitors verapamil , DL-AP5 and MCPG , respectively .
	manualset3
90964	1	399130	13	NULL	NULL	0	NULL	Hyperpolarization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperpolarization was accompanied by a concomitant decrease in the membrane input resistance ( control = 16.6 + / - 2.8 Momega ; 10 ( -4 ) M 5-HT = 6.4 + / - 1.3 MD ; n = 6 , P & lt ; 0.05 ) and time constant ( control = 60.3 + / - 13.1 ms ; 10 ( -4 ) M 5-HT = 16.0 + / - 4.4 ms , n = 6 , P & lt ; 0.05 ) .
	manualset3
90965	2	399130	13	NULL	NULL	0	NULL	membrane input resistance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperpolarization was accompanied by a concomitant decrease in the membrane input resistance ( control = 16.6 + / - 2.8 Momega ; 10 ( -4 ) M 5-HT = 6.4 + / - 1.3 MD ; n = 6 , P & lt ; 0.05 ) and time constant ( control = 60.3 + / - 13.1 ms ; 10 ( -4 ) M 5-HT = 16.0 + / - 4.4 ms , n = 6 , P & lt ; 0.05 ) .
	manualset3
90966	3	399130	13	NULL	NULL	0	NULL	control = 16.6 + / - 2.8 Momega ; 10 ( -4 ) M 5-HT = 6.4 + / - 1.3 MD ; n = 6 , P & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperpolarization was accompanied by a concomitant decrease in the membrane input resistance ( control = 16.6 + / - 2.8 Momega ; 10 ( -4 ) M 5-HT = 6.4 + / - 1.3 MD ; n = 6 , P & lt ; 0.05 ) and time constant ( control = 60.3 + / - 13.1 ms ; 10 ( -4 ) M 5-HT = 16.0 + / - 4.4 ms , n = 6 , P & lt ; 0.05 ) .
	manualset3
90967	4	399130	13	NULL	NULL	0	NULL	time constant ( control = 60.3 + / - 13.1 ms ; 10 ( -4 ) M 5-HT = 16.0 + / - 4.4 ms , n = 6 , P & lt ; 0.05 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperpolarization was accompanied by a concomitant decrease in the membrane input resistance ( control = 16.6 + / - 2.8 Momega ; 10 ( -4 ) M 5-HT = 6.4 + / - 1.3 MD ; n = 6 , P & lt ; 0.05 ) and time constant ( control = 60.3 + / - 13.1 ms ; 10 ( -4 ) M 5-HT = 16.0 + / - 4.4 ms , n = 6 , P & lt ; 0.05 ) .
	manualset3
91092	1	399131	13	NULL	NULL	0	NULL	Hypertension-dependent cerebrovascular changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypertension-dependent cerebrovascular changes were documented primarily in brain pial arteries , whereas no information is so far available concerning changes of peripheral nerve vascularization in hypertension .
	manualset3
91093	2	399131	13	NULL	NULL	0	NULL	brain pial arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypertension-dependent cerebrovascular changes were documented primarily in brain pial arteries , whereas no information is so far available concerning changes of peripheral nerve vascularization in hypertension .
	manualset3
91094	3	399131	13	NULL	NULL	0	NULL	information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypertension-dependent cerebrovascular changes were documented primarily in brain pial arteries , whereas no information is so far available concerning changes of peripheral nerve vascularization in hypertension .
	manualset3
91095	4	399131	13	NULL	NULL	0	NULL	changes of peripheral nerve vascularization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypertension-dependent cerebrovascular changes were documented primarily in brain pial arteries , whereas no information is so far available concerning changes of peripheral nerve vascularization in hypertension .
	manualset3
91096	5	399131	13	NULL	NULL	0	NULL	hypertension 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypertension-dependent cerebrovascular changes were documented primarily in brain pial arteries , whereas no information is so far available concerning changes of peripheral nerve vascularization in hypertension .
	manualset3
91097	1	399132	13	NULL	NULL	0	NULL	Hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypertension is very prevalent in chronic kidney disease and critical for its prognosis .
	manualset3
91098	2	399132	13	NULL	NULL	0	NULL	chronic kidney disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypertension is very prevalent in chronic kidney disease and critical for its prognosis .
	manualset3
91099	3	399132	13	NULL	NULL	0	NULL	prognosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypertension is very prevalent in chronic kidney disease and critical for its prognosis .
	manualset3
91100	1	399133	13	NULL	NULL	0	NULL	Hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypertension remains the most common complication associated with cyclosporine administration in heart transplant recipients .
	manualset3
91101	2	399133	13	NULL	NULL	0	NULL	complication 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypertension remains the most common complication associated with cyclosporine administration in heart transplant recipients .
	manualset3
91102	3	399133	13	NULL	NULL	0	NULL	cyclosporine administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypertension remains the most common complication associated with cyclosporine administration in heart transplant recipients .
	manualset3
91103	4	399133	13	NULL	NULL	0	NULL	heart transplant recipients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypertension remains the most common complication associated with cyclosporine administration in heart transplant recipients .
	manualset3
91104	1	399134	13	NULL	NULL	0	NULL	partial thickness facial burns 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypertrophic scarring after partial thickness facial burns is common when epithelialization takes longer than 3 weeks .
	manualset3
91105	2	399134	13	NULL	NULL	0	NULL	epithelialization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypertrophic scarring after partial thickness facial burns is common when epithelialization takes longer than 3 weeks .
	manualset3
91106	3	399134	13	NULL	NULL	0	NULL	3 weeks 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypertrophic scarring after partial thickness facial burns is common when epithelialization takes longer than 3 weeks .
	manualset3
98569	4	399134	13	NULL	NULL	0	NULL	Hypertrophic scarring	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypertrophic scarring after partial thickness facial burns is common when epithelialization takes longer than 3 weeks .
	manualset3
91107	1	399135	13	NULL	NULL	0	NULL	Hyperuricemic nephropathy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperuricemic nephropathy can progress to the permanent renal damage even in infancy in partial hypoxanthine-guanine phosphoribosyltransferase ( HPRT ) deficiency .
	manualset3
91108	2	399135	13	NULL	NULL	0	NULL	progress 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperuricemic nephropathy can progress to the permanent renal damage even in infancy in partial hypoxanthine-guanine phosphoribosyltransferase ( HPRT ) deficiency .
	manualset3
91109	3	399135	13	NULL	NULL	0	NULL	permanent renal damage 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperuricemic nephropathy can progress to the permanent renal damage even in infancy in partial hypoxanthine-guanine phosphoribosyltransferase ( HPRT ) deficiency .
	manualset3
91110	4	399135	13	NULL	NULL	0	NULL	infancy	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperuricemic nephropathy can progress to the permanent renal damage even in infancy in partial hypoxanthine-guanine phosphoribosyltransferase ( HPRT ) deficiency .
	manualset3
91111	5	399135	13	NULL	NULL	0	NULL	 partial hypoxanthine-guanine phosphoribosyltransferase ( HPRT ) deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyperuricemic nephropathy can progress to the permanent renal damage even in infancy in partial hypoxanthine-guanine phosphoribosyltransferase ( HPRT ) deficiency .
	manualset3
91112	1	399136	13	NULL	NULL	0	NULL	Hypnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypnosis using a communication device to increase magnetic resonance imaging tolerance with a claustrophobic patient .
	manualset3
91113	2	399136	13	NULL	NULL	0	NULL	communication device	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypnosis using a communication device to increase magnetic resonance imaging tolerance with a claustrophobic patient .
	manualset3
91114	3	399136	13	NULL	NULL	0	NULL	magnetic resonance imaging tolerance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypnosis using a communication device to increase magnetic resonance imaging tolerance with a claustrophobic patient .
	manualset3
91115	4	399136	13	NULL	NULL	0	NULL	claustrophobic patient	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypnosis using a communication device to increase magnetic resonance imaging tolerance with a claustrophobic patient .
	manualset3
91116	1	399137	13	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	( The relationship between occupational stress and serum glycosylated hemoglobin A1c level ) .
	manualset3
91117	2	399137	13	NULL	NULL	0	NULL	occupational stress	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	( The relationship between occupational stress and serum glycosylated hemoglobin A1c level ) .
	manualset3
91118	3	399137	13	NULL	NULL	0	NULL	serum glycosylated hemoglobin A1c level	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( The relationship between occupational stress and serum glycosylated hemoglobin A1c level ) .
	manualset3
91119	1	399138	13	NULL	NULL	0	NULL	Hypobaric-hypoxic exposure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypobaric-hypoxic exposure and histochemical responses of soleus muscle fibers in the rat .
	manualset3
91120	2	399138	13	NULL	NULL	0	NULL	histochemical responses 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypobaric-hypoxic exposure and histochemical responses of soleus muscle fibers in the rat .
	manualset3
91121	3	399138	13	NULL	NULL	0	NULL	soleus muscle fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypobaric-hypoxic exposure and histochemical responses of soleus muscle fibers in the rat .
	manualset3
91122	4	399138	13	NULL	NULL	0	NULL	rat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypobaric-hypoxic exposure and histochemical responses of soleus muscle fibers in the rat .
	manualset3
91123	1	399139	13	NULL	NULL	0	NULL	Hypocalcemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypocalcemia after intravenous bisphosphonate : lesson to be learned .
	manualset3
91124	2	399139	13	NULL	NULL	0	NULL	intravenous bisphosphonate	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypocalcemia after intravenous bisphosphonate : lesson to be learned .
	manualset3
91125	3	399139	13	NULL	NULL	0	NULL	lesson	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypocalcemia after intravenous bisphosphonate : lesson to be learned .
	manualset3
91126	1	399140	13	NULL	NULL	0	NULL	Hypocalcemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypocalcemia in metastatic bone disease : metabolic and radionuclide studies of a case .
	manualset3
91127	2	399140	13	NULL	NULL	0	NULL	metastatic bone disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypocalcemia in metastatic bone disease : metabolic and radionuclide studies of a case .
	manualset3
91128	3	399140	13	NULL	NULL	0	NULL	 metabolic studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypocalcemia in metastatic bone disease : metabolic and radionuclide studies of a case .
	manualset3
91129	4	399140	13	NULL	NULL	0	NULL	radionuclide studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypocalcemia in metastatic bone disease : metabolic and radionuclide studies of a case .
	manualset3
91130	5	399140	13	NULL	NULL	NULL	NULL	 case	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hypocalcemia in metastatic bone disease : metabolic and radionuclide studies of a case .
	manualset3
91131	1	399141	13	NULL	NULL	0	NULL	Hypochaeris 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypochaeris ( consisting of H. glabra , H. radicata , H. arachnoidea , and H. salzmanniana ) .
	manualset3
91132	2	399141	13	NULL	NULL	0	NULL	H. glabra	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypochaeris ( consisting of H. glabra , H. radicata , H. arachnoidea , and H. salzmanniana ) .
	manualset3
91133	3	399141	13	NULL	NULL	0	NULL	H. radicata	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypochaeris ( consisting of H. glabra , H. radicata , H. arachnoidea , and H. salzmanniana ) .
	manualset3
91134	4	399141	13	NULL	NULL	0	NULL	H. arachnoidea	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypochaeris ( consisting of H. glabra , H. radicata , H. arachnoidea , and H. salzmanniana ) .
	manualset3
91135	5	399141	13	NULL	NULL	0	NULL	H. salzmanniana 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypochaeris ( consisting of H. glabra , H. radicata , H. arachnoidea , and H. salzmanniana ) .
	manualset3
91136	1	399142	13	NULL	NULL	0	NULL	Hypohidrotic ectodermal dysplasia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypohidrotic ectodermal dysplasia : a genealogic , stereomicroscope , and scanning electron microscope study .
	manualset3
91137	2	399142	13	NULL	NULL	0	NULL	genealogic study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypohidrotic ectodermal dysplasia : a genealogic , stereomicroscope , and scanning electron microscope study .
	manualset3
91138	3	399142	13	NULL	NULL	0	NULL	 stereomicroscope study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypohidrotic ectodermal dysplasia : a genealogic , stereomicroscope , and scanning electron microscope study .
	manualset3
91139	4	399142	13	NULL	NULL	0	NULL	scanning electron microscope study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypohidrotic ectodermal dysplasia : a genealogic , stereomicroscope , and scanning electron microscope study .
	manualset3
91140	1	399143	13	NULL	NULL	0	NULL	Hyporeflexia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyporeflexia in workers chronically exposed to organophosphate insecticides .
	manualset3
91141	2	399143	13	NULL	NULL	0	NULL	workers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyporeflexia in workers chronically exposed to organophosphate insecticides .
	manualset3
91142	3	399143	13	NULL	NULL	0	NULL	organophosphate insecticides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hyporeflexia in workers chronically exposed to organophosphate insecticides .
	manualset3
91143	1	399144	13	NULL	NULL	0	NULL	Hypothalamic ER mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothalamic ER mRNA was decreased in response to melatonin in both intact and ovariectomized animals by 25 % .
	manualset3
91144	2	399144	13	NULL	NULL	0	NULL	response to melatonin 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothalamic ER mRNA was decreased in response to melatonin in both intact and ovariectomized animals by 25 % .
	manualset3
91145	3	399144	13	NULL	NULL	0	NULL	intact animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothalamic ER mRNA was decreased in response to melatonin in both intact and ovariectomized animals by 25 % .
	manualset3
91146	4	399144	13	NULL	NULL	0	NULL	ovariectomized animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothalamic ER mRNA was decreased in response to melatonin in both intact and ovariectomized animals by 25 % .
	manualset3
91147	5	399144	13	NULL	NULL	0	NULL	25 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothalamic ER mRNA was decreased in response to melatonin in both intact and ovariectomized animals by 25 % .
	manualset3
91148	1	399145	13	NULL	NULL	0	NULL	Hypothalamic blood flow	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothalamic blood flow remains unaltered following chronic nitric oxide synthase blockade in rats .
	manualset3
91149	2	399145	13	NULL	NULL	0	NULL	chronic nitric oxide synthase blockade	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothalamic blood flow remains unaltered following chronic nitric oxide synthase blockade in rats .
	manualset3
91150	3	399145	13	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothalamic blood flow remains unaltered following chronic nitric oxide synthase blockade in rats .
	manualset3
91151	1	399146	13	NULL	NULL	0	NULL	Hypothalamic preparations	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothalamic preparations exhibited the greatest insulin binding .
	manualset3
91152	2	399146	13	NULL	NULL	0	NULL	insulin binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothalamic preparations exhibited the greatest insulin binding .
	manualset3
91153	1	399147	13	NULL	NULL	0	NULL	nitric oxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( The release of nitric oxide from organic nitroso compounds in the body of animals ) .
	manualset3
91154	2	399147	13	NULL	NULL	0	NULL	organic nitroso compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( The release of nitric oxide from organic nitroso compounds in the body of animals ) .
	manualset3
91155	3	399147	13	NULL	NULL	NULL	NULL	body of animals	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The release of nitric oxide from organic nitroso compounds in the body of animals ) .
	manualset3
91156	1	399148	13	NULL	NULL	0	NULL	Hypothermic preservation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothermic preservation effect on mammalian cells of type III antifreeze proteins from notched-fin eelpout .
	manualset3
91157	2	399148	13	NULL	NULL	NULL	NULL	effect	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hypothermic preservation effect on mammalian cells of type III antifreeze proteins from notched-fin eelpout .
	manualset3
91158	3	399148	13	NULL	NULL	0	NULL	 mammalian cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothermic preservation effect on mammalian cells of type III antifreeze proteins from notched-fin eelpout .
	manualset3
91159	4	399148	13	NULL	NULL	0	NULL	type III antifreeze proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothermic preservation effect on mammalian cells of type III antifreeze proteins from notched-fin eelpout .
	manualset3
91160	5	399148	13	NULL	NULL	0	NULL	notched-fin eelpout	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothermic preservation effect on mammalian cells of type III antifreeze proteins from notched-fin eelpout .
	manualset3
91161	1	399149	13	NULL	NULL	0	NULL	Hypotheses	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypotheses were : ( a ) the quality of mother-daughter attachment will mediate the relationship between their social support and drug use and ( b ) the effects of mothers ' and daughters ' chronic stress on their drug use is mediated by their social support which , in turn , is also mediated by the quality of their attachment after taking into account socio-demographic variables .
	manualset3
91163	3	399149	13	NULL	NULL	NULL	NULL	quality of mother-daughter attachment	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hypotheses were : ( a ) the quality of mother-daughter attachment will mediate the relationship between their social support and drug use and ( b ) the effects of mothers ' and daughters ' chronic stress on their drug use is mediated by their social support which , in turn , is also mediated by the quality of their attachment after taking into account socio-demographic variables .
	manualset3
91164	4	399149	13	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypotheses were : ( a ) the quality of mother-daughter attachment will mediate the relationship between their social support and drug use and ( b ) the effects of mothers ' and daughters ' chronic stress on their drug use is mediated by their social support which , in turn , is also mediated by the quality of their attachment after taking into account socio-demographic variables .
	manualset3
91165	5	399149	13	NULL	NULL	NULL	NULL	drug use	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hypotheses were : ( a ) the quality of mother-daughter attachment will mediate the relationship between their social support and drug use and ( b ) the effects of mothers ' and daughters ' chronic stress on their drug use is mediated by their social support which , in turn , is also mediated by the quality of their attachment after taking into account socio-demographic variables .
	manualset3
91166	6	399149	13	NULL	NULL	0	NULL	effects of mothers ' and daughters ' chronic stress 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypotheses were : ( a ) the quality of mother-daughter attachment will mediate the relationship between their social support and drug use and ( b ) the effects of mothers ' and daughters ' chronic stress on their drug use is mediated by their social support which , in turn , is also mediated by the quality of their attachment after taking into account socio-demographic variables .
	manualset3
91167	7	399149	13	NULL	NULL	NULL	NULL	drug use	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hypotheses were : ( a ) the quality of mother-daughter attachment will mediate the relationship between their social support and drug use and ( b ) the effects of mothers ' and daughters ' chronic stress on their drug use is mediated by their social support which , in turn , is also mediated by the quality of their attachment after taking into account socio-demographic variables .
	manualset3
91168	8	399149	13	NULL	NULL	0	NULL	quality of their attachment 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypotheses were : ( a ) the quality of mother-daughter attachment will mediate the relationship between their social support and drug use and ( b ) the effects of mothers ' and daughters ' chronic stress on their drug use is mediated by their social support which , in turn , is also mediated by the quality of their attachment after taking into account socio-demographic variables .
	manualset3
91169	9	399149	13	NULL	NULL	NULL	NULL	socio-demographic variables	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hypotheses were : ( a ) the quality of mother-daughter attachment will mediate the relationship between their social support and drug use and ( b ) the effects of mothers ' and daughters ' chronic stress on their drug use is mediated by their social support which , in turn , is also mediated by the quality of their attachment after taking into account socio-demographic variables .
	manualset3
98570	10	399149	13	NULL	NULL	0	NULL	social support	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypotheses were : ( a ) the quality of mother-daughter attachment will mediate the relationship between their social support and drug use and ( b ) the effects of mothers ' and daughters ' chronic stress on their drug use is mediated by their social support which , in turn , is also mediated by the quality of their attachment after taking into account socio-demographic variables .
	manualset3
91170	1	399150	13	NULL	NULL	0	NULL	Hypothesis 3 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothesis 3 did not contribute to the explanation of forest age effects on NEP .
	manualset3
91171	2	399150	13	NULL	NULL	0	NULL	explanation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothesis 3 did not contribute to the explanation of forest age effects on NEP .
	manualset3
91172	3	399150	13	NULL	NULL	0	NULL	forest age effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothesis 3 did not contribute to the explanation of forest age effects on NEP .
	manualset3
91173	4	399150	13	NULL	NULL	0	NULL	NEP 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothesis 3 did not contribute to the explanation of forest age effects on NEP .
	manualset3
91174	1	399151	13	NULL	NULL	0	NULL	Hypothyroid larvae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothyroid larvae were produced by rearing the animals , beginning at stage 48 , in a 0.01 % solution of propylthiouracil ( PTU ) , a treatment that blocks synthesis of thyroid hormone .
	manualset3
91175	2	399151	13	NULL	NULL	0	NULL	animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothyroid larvae were produced by rearing the animals , beginning at stage 48 , in a 0.01 % solution of propylthiouracil ( PTU ) , a treatment that blocks synthesis of thyroid hormone .
	manualset3
91176	3	399151	13	NULL	NULL	0	NULL	stage 48	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothyroid larvae were produced by rearing the animals , beginning at stage 48 , in a 0.01 % solution of propylthiouracil ( PTU ) , a treatment that blocks synthesis of thyroid hormone .
	manualset3
91177	4	399151	13	NULL	NULL	0	NULL	0.01 % solution	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothyroid larvae were produced by rearing the animals , beginning at stage 48 , in a 0.01 % solution of propylthiouracil ( PTU ) , a treatment that blocks synthesis of thyroid hormone .
	manualset3
91178	5	399151	13	NULL	NULL	0	NULL	 propylthiouracil ( PTU )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothyroid larvae were produced by rearing the animals , beginning at stage 48 , in a 0.01 % solution of propylthiouracil ( PTU ) , a treatment that blocks synthesis of thyroid hormone .
	manualset3
91179	6	399151	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothyroid larvae were produced by rearing the animals , beginning at stage 48 , in a 0.01 % solution of propylthiouracil ( PTU ) , a treatment that blocks synthesis of thyroid hormone .
	manualset3
91180	7	399151	13	NULL	NULL	NULL	NULL	synthesis of thyroid hormone	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hypothyroid larvae were produced by rearing the animals , beginning at stage 48 , in a 0.01 % solution of propylthiouracil ( PTU ) , a treatment that blocks synthesis of thyroid hormone .
	manualset3
91181	1	399152	13	NULL	NULL	0	NULL	Hypothyroidism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothyroidism is a typical low rennin HT form showing a better antihypertensive response to CCB and diuretics ; indeed in hypothyroidism a low-sodium diet seems further to improve BP control .
	manualset3
91182	2	399152	13	NULL	NULL	0	NULL	low rennin HT	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothyroidism is a typical low rennin HT form showing a better antihypertensive response to CCB and diuretics ; indeed in hypothyroidism a low-sodium diet seems further to improve BP control .
	manualset3
91183	3	399152	13	NULL	NULL	0	NULL	antihypertensive response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothyroidism is a typical low rennin HT form showing a better antihypertensive response to CCB and diuretics ; indeed in hypothyroidism a low-sodium diet seems further to improve BP control .
	manualset3
91184	4	399152	13	NULL	NULL	0	NULL	 CCB	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothyroidism is a typical low rennin HT form showing a better antihypertensive response to CCB and diuretics ; indeed in hypothyroidism a low-sodium diet seems further to improve BP control .
	manualset3
91185	5	399152	13	NULL	NULL	0	NULL	diuretics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothyroidism is a typical low rennin HT form showing a better antihypertensive response to CCB and diuretics ; indeed in hypothyroidism a low-sodium diet seems further to improve BP control .
	manualset3
91186	6	399152	13	NULL	NULL	0	NULL	hypothyroidism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothyroidism is a typical low rennin HT form showing a better antihypertensive response to CCB and diuretics ; indeed in hypothyroidism a low-sodium diet seems further to improve BP control .
	manualset3
91187	7	399152	13	NULL	NULL	0	NULL	low-sodium diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothyroidism is a typical low rennin HT form showing a better antihypertensive response to CCB and diuretics ; indeed in hypothyroidism a low-sodium diet seems further to improve BP control .
	manualset3
91188	8	399152	13	NULL	NULL	0	NULL	BP	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothyroidism is a typical low rennin HT form showing a better antihypertensive response to CCB and diuretics ; indeed in hypothyroidism a low-sodium diet seems further to improve BP control .
	manualset3
91189	1	399153	13	NULL	NULL	0	NULL	Hypoxia-induced acidosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypoxia-induced acidosis uncouples the STIM-Orai calcium signaling complex .
	manualset3
91190	2	399153	13	NULL	NULL	0	NULL	STIM-Orai calcium signaling complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypoxia-induced acidosis uncouples the STIM-Orai calcium signaling complex .
	manualset3
91191	1	399154	13	NULL	NULL	0	NULL	Hypoxia-induced expression of C1q	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypoxia-induced expression of C1q , a subcomponent of the complement system , in cultured rat PC12 cells .
	manualset3
91192	2	399154	13	NULL	NULL	0	NULL	a subcomponent of the complement system	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypoxia-induced expression of C1q , a subcomponent of the complement system , in cultured rat PC12 cells .
	manualset3
91193	3	399154	13	NULL	NULL	0	NULL	cultured rat PC12 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypoxia-induced expression of C1q , a subcomponent of the complement system , in cultured rat PC12 cells .
	manualset3
91194	1	399155	13	NULL	NULL	0	NULL	Hypoxia-induced suppression of automaticity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypoxia-induced suppression of automaticity was reversed completely by 5 mM glucose , and partially by 40 mM valine .
	manualset3
91195	2	399155	13	NULL	NULL	0	NULL	5 mM glucose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypoxia-induced suppression of automaticity was reversed completely by 5 mM glucose , and partially by 40 mM valine .
	manualset3
91196	3	399155	13	NULL	NULL	0	NULL	40 mM valine	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypoxia-induced suppression of automaticity was reversed completely by 5 mM glucose , and partially by 40 mM valine .
	manualset3
91197	1	399156	13	NULL	NULL	NULL	NULL	Hypoxia inducible factor ( HIF ) 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hypoxia inducible factor ( HIF ) , the most potent regulator of VEGF , is a heterodimer of a constitutively expressed beta subunit and an oxygen-regulated alpha subunit ( HIF-alpha ) .
	manualset3
91198	2	399156	13	NULL	NULL	NULL	NULL	 regulator of VEGF 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hypoxia inducible factor ( HIF ) , the most potent regulator of VEGF , is a heterodimer of a constitutively expressed beta subunit and an oxygen-regulated alpha subunit ( HIF-alpha ) .
	manualset3
91199	3	399156	13	NULL	NULL	NULL	NULL	heterodimer	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hypoxia inducible factor ( HIF ) , the most potent regulator of VEGF , is a heterodimer of a constitutively expressed beta subunit and an oxygen-regulated alpha subunit ( HIF-alpha ) .
	manualset3
91200	4	399156	13	NULL	NULL	0	NULL	beta subunit	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypoxia inducible factor ( HIF ) , the most potent regulator of VEGF , is a heterodimer of a constitutively expressed beta subunit and an oxygen-regulated alpha subunit ( HIF-alpha ) .
	manualset3
91201	5	399156	13	NULL	NULL	0	NULL	xygen-regulated alpha subunit ( HIF-alpha )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypoxia inducible factor ( HIF ) , the most potent regulator of VEGF , is a heterodimer of a constitutively expressed beta subunit and an oxygen-regulated alpha subunit ( HIF-alpha ) .
	manualset3
91202	1	399157	13	NULL	NULL	NULL	NULL	Hypoxia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hypoxia was determined biochemically by ATP and phosphocreatine ( PCr ) levels .
	manualset3
91203	2	399157	13	NULL	NULL	0	NULL	ATP levels  	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypoxia was determined biochemically by ATP and phosphocreatine ( PCr ) levels .
	manualset3
91204	3	399157	13	NULL	NULL	0	NULL	phosphocreatine ( PCr ) levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypoxia was determined biochemically by ATP and phosphocreatine ( PCr ) levels .
	manualset3
91205	1	399158	13	NULL	NULL	0	NULL	I-cell disease ( mucolipidosis II ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	I-cell disease ( mucolipidosis II ) is a fatal childhood disorder affecting the expression of multiple lysosomal acid hydrolases .
	manualset3
91206	2	399158	13	NULL	NULL	0	NULL	fatal childhood disorder	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	I-cell disease ( mucolipidosis II ) is a fatal childhood disorder affecting the expression of multiple lysosomal acid hydrolases .
	manualset3
91207	3	399158	13	NULL	NULL	0	NULL	expression of multiple lysosomal acid hydrolases	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	I-cell disease ( mucolipidosis II ) is a fatal childhood disorder affecting the expression of multiple lysosomal acid hydrolases .
	manualset3
91208	1	399159	13	NULL	NULL	0	NULL	Antigenic differences	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Antigenic differences between parasite lines detected by crossed immunoelectrophoresis .
	manualset3
91209	2	399159	13	NULL	NULL	0	NULL	parasite lines	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Antigenic differences between parasite lines detected by crossed immunoelectrophoresis .
	manualset3
91210	3	399159	13	NULL	NULL	0	NULL	crossed immunoelectrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Antigenic differences between parasite lines detected by crossed immunoelectrophoresis .
	manualset3
90393	1	399160	13	NULL	NULL	NULL	NULL	Dependence 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	I. Dependence on composition of the configurational stability of deoxyribonucleic acids .
	manualset3
91241	2	399160	13	NULL	NULL	0	NULL	composition	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Dependence on composition of the configurational stability of deoxyribonucleic acids .
	manualset3
91242	3	399160	13	NULL	NULL	0	NULL	configurational stability 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Dependence on composition of the configurational stability of deoxyribonucleic acids .
	manualset3
91243	4	399160	13	NULL	NULL	0	NULL	 deoxyribonucleic acids 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Dependence on composition of the configurational stability of deoxyribonucleic acids .
	manualset3
91244	1	399161	13	NULL	NULL	0	NULL	Differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Differences in reactivity with Poly ( U ) and Poly - ( A ) Poly ( U ) .
	manualset3
91245	2	399161	13	NULL	NULL	0	NULL	reactivity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Differences in reactivity with Poly ( U ) and Poly - ( A ) Poly ( U ) .
	manualset3
91246	3	399161	13	NULL	NULL	0	NULL	Poly ( U )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Differences in reactivity with Poly ( U ) and Poly - ( A ) Poly ( U ) .
	manualset3
91247	4	399161	13	NULL	NULL	0	NULL	Poly - ( A ) Poly ( U )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Differences in reactivity with Poly ( U ) and Poly - ( A ) Poly ( U ) .
	manualset3
91248	1	399162	13	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( The role of B72 .3 125-I monoclonal antibody in the radioimmunoguided surgery of colorectal neoplasms ) .
	manualset3
91249	2	399162	13	NULL	NULL	0	NULL	B72 .3 125-I monoclonal antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( The role of B72 .3 125-I monoclonal antibody in the radioimmunoguided surgery of colorectal neoplasms ) .
	manualset3
91250	3	399162	13	NULL	NULL	0	NULL	radioimmunoguided surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( The role of B72 .3 125-I monoclonal antibody in the radioimmunoguided surgery of colorectal neoplasms ) .
	manualset3
91251	4	399162	13	NULL	NULL	0	NULL	colorectal neoplasms	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( The role of B72 .3 125-I monoclonal antibody in the radioimmunoguided surgery of colorectal neoplasms ) .
	manualset3
91252	1	399163	13	NULL	NULL	0	NULL	Effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Effect of 8-methoxypsoralen on the epidermal patch test in allergic contact eczema ) .
	manualset3
91253	2	399163	13	NULL	NULL	0	NULL	8-methoxypsoralen	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Effect of 8-methoxypsoralen on the epidermal patch test in allergic contact eczema ) .
	manualset3
91254	3	399163	13	NULL	NULL	0	NULL	epidermal patch test	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Effect of 8-methoxypsoralen on the epidermal patch test in allergic contact eczema ) .
	manualset3
91255	4	399163	13	NULL	NULL	0	NULL	allergic contact eczema	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Effect of 8-methoxypsoralen on the epidermal patch test in allergic contact eczema ) .
	manualset3
91256	1	399164	13	NULL	NULL	0	NULL	Isolation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Isolation and characterization of the virus .
	manualset3
91257	2	399164	13	NULL	NULL	0	NULL	characterization 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Isolation and characterization of the virus .
	manualset3
91258	3	399164	13	NULL	NULL	0	NULL	virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Isolation and characterization of the virus .
	manualset3
91259	1	399165	13	NULL	NULL	0	NULL	Observations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Observations on H 10 Z tumor short term tissue cultures .
	manualset3
91260	2	399165	13	NULL	NULL	0	NULL	H 10 Z tumor short term tissue cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Observations on H 10 Z tumor short term tissue cultures .
	manualset3
91261	1	399166	13	NULL	NULL	NULL	NULL	Regional fibrinolysis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	I. Regional fibrinolysis ( cerebral , of the upper extremity and of the lower extremity ) caused by `` arterial '' administration of nicotinic acid ) .
	manualset3
91262	2	399166	13	NULL	NULL	0	NULL	 cerebral , of the upper extremity	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Regional fibrinolysis ( cerebral , of the upper extremity and of the lower extremity ) caused by `` arterial '' administration of nicotinic acid ) .
	manualset3
91263	3	399166	13	NULL	NULL	0	NULL	cerebral of the lower extremity	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Regional fibrinolysis ( cerebral , of the upper extremity and of the lower extremity ) caused by `` arterial '' administration of nicotinic acid ) .
	manualset3
91264	4	399166	13	NULL	NULL	NULL	NULL	`` arterial '' administration	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	I. Regional fibrinolysis ( cerebral , of the upper extremity and of the lower extremity ) caused by `` arterial '' administration of nicotinic acid ) .
	manualset3
91265	5	399166	13	NULL	NULL	0	NULL	nicotinic acid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Regional fibrinolysis ( cerebral , of the upper extremity and of the lower extremity ) caused by `` arterial '' administration of nicotinic acid ) .
	manualset3
91266	1	399167	13	NULL	NULL	0	NULL	Cytological changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Cytological changes associated with the exposure of Escherichia coli to colistin sulfate .
	manualset3
91267	2	399167	13	NULL	NULL	0	NULL	exposure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Cytological changes associated with the exposure of Escherichia coli to colistin sulfate .
	manualset3
91268	3	399167	13	NULL	NULL	0	NULL	Escherichia coli 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Cytological changes associated with the exposure of Escherichia coli to colistin sulfate .
	manualset3
91269	4	399167	13	NULL	NULL	0	NULL	colistin sulfate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Cytological changes associated with the exposure of Escherichia coli to colistin sulfate .
	manualset3
91270	1	399168	13	NULL	NULL	0	NULL	T-T interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Collaborative T-T interactions in the immunoregulation of B cell differentiation .
	manualset3
91271	2	399168	13	NULL	NULL	0	NULL	 immunoregulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Collaborative T-T interactions in the immunoregulation of B cell differentiation .
	manualset3
91272	3	399168	13	NULL	NULL	0	NULL	B cell differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Collaborative T-T interactions in the immunoregulation of B cell differentiation .
	manualset3
91273	1	399169	13	NULL	NULL	0	NULL	 role 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( The role of D2 lymphadenectomy in the surgical treatment of gastric carcinoma ) .
	manualset3
91274	2	399169	13	NULL	NULL	0	NULL	D2 lymphadenectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( The role of D2 lymphadenectomy in the surgical treatment of gastric carcinoma ) .
	manualset3
91275	3	399169	13	NULL	NULL	0	NULL	surgical treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( The role of D2 lymphadenectomy in the surgical treatment of gastric carcinoma ) .
	manualset3
91276	4	399169	13	NULL	NULL	0	NULL	gastric carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( The role of D2 lymphadenectomy in the surgical treatment of gastric carcinoma ) .
	manualset3
91277	1	399170	13	NULL	NULL	0	NULL	Clinical studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Clinical and statistical studies on the effect of dentition on the hearing organ and hearing in 5000 patients treated in an otolaryngologic clinic ) .
	manualset3
91278	2	399170	13	NULL	NULL	0	NULL	statistical studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Clinical and statistical studies on the effect of dentition on the hearing organ and hearing in 5000 patients treated in an otolaryngologic clinic ) .
	manualset3
91279	3	399170	13	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Clinical and statistical studies on the effect of dentition on the hearing organ and hearing in 5000 patients treated in an otolaryngologic clinic ) .
	manualset3
91280	4	399170	13	NULL	NULL	0	NULL	dentition 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Clinical and statistical studies on the effect of dentition on the hearing organ and hearing in 5000 patients treated in an otolaryngologic clinic ) .
	manualset3
91281	5	399170	13	NULL	NULL	0	NULL	hearing organ 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Clinical and statistical studies on the effect of dentition on the hearing organ and hearing in 5000 patients treated in an otolaryngologic clinic ) .
	manualset3
91282	6	399170	13	NULL	NULL	0	NULL	 hearing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Clinical and statistical studies on the effect of dentition on the hearing organ and hearing in 5000 patients treated in an otolaryngologic clinic ) .
	manualset3
91283	7	399170	13	NULL	NULL	0	NULL	5000	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Clinical and statistical studies on the effect of dentition on the hearing organ and hearing in 5000 patients treated in an otolaryngologic clinic ) .
	manualset3
91284	8	399170	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Clinical and statistical studies on the effect of dentition on the hearing organ and hearing in 5000 patients treated in an otolaryngologic clinic ) .
	manualset3
91285	9	399170	13	NULL	NULL	0	NULL	otolaryngologic clinic	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Clinical and statistical studies on the effect of dentition on the hearing organ and hearing in 5000 patients treated in an otolaryngologic clinic ) .
	manualset3
91286	1	399171	13	NULL	NULL	NULL	NULL	Alterations 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	I. Alterations in the metabolism of xenobiotic compounds and D-glucuronic acid pathway .
	manualset3
91287	2	399171	13	NULL	NULL	0	NULL	metabolism of xenobiotic compounds	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Alterations in the metabolism of xenobiotic compounds and D-glucuronic acid pathway .
	manualset3
91288	3	399171	13	NULL	NULL	0	NULL	D-glucuronic acid pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Alterations in the metabolism of xenobiotic compounds and D-glucuronic acid pathway .
	manualset3
91289	1	399172	13	NULL	NULL	0	NULL	 Development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Development of collicular responses to optic stimulation ) .
	manualset3
91290	2	399172	13	NULL	NULL	0	NULL	collicular responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Development of collicular responses to optic stimulation ) .
	manualset3
91291	3	399172	13	NULL	NULL	0	NULL	optic stimulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Development of collicular responses to optic stimulation ) .
	manualset3
91292	1	399173	13	NULL	NULL	0	NULL	( vti ) 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	I ( vti ) showed a half-maximal activation around -102 mV with a slope factor of 25 mV .
	manualset3
91293	2	399173	13	NULL	NULL	0	NULL	half-maximal activation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	I ( vti ) showed a half-maximal activation around -102 mV with a slope factor of 25 mV .
	manualset3
91294	3	399173	13	NULL	NULL	0	NULL	-102 mV 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	I ( vti ) showed a half-maximal activation around -102 mV with a slope factor of 25 mV .
	manualset3
91295	4	399173	13	NULL	NULL	0	NULL	slope factor of 25 mV	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	I ( vti ) showed a half-maximal activation around -102 mV with a slope factor of 25 mV .
	manualset3
91296	1	399174	13	NULL	NULL	0	NULL	present issue of Current Drug Targets	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	I guest-edited the present issue of Current Drug Targets aiming to bring together a number of leading experts in the field of cancer chemoprevention , who would systematically review the evidence ; discuss the clinical and experimental data ; highlight new approaches and promising directions for future research .
	manualset3
91297	2	399174	13	NULL	NULL	0	NULL	number of leading experts	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	I guest-edited the present issue of Current Drug Targets aiming to bring together a number of leading experts in the field of cancer chemoprevention , who would systematically review the evidence ; discuss the clinical and experimental data ; highlight new approaches and promising directions for future research .
	manualset3
91298	3	399174	13	NULL	NULL	0	NULL	field of cancer chemoprevention	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	I guest-edited the present issue of Current Drug Targets aiming to bring together a number of leading experts in the field of cancer chemoprevention , who would systematically review the evidence ; discuss the clinical and experimental data ; highlight new approaches and promising directions for future research .
	manualset3
91299	4	399174	13	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	I guest-edited the present issue of Current Drug Targets aiming to bring together a number of leading experts in the field of cancer chemoprevention , who would systematically review the evidence ; discuss the clinical and experimental data ; highlight new approaches and promising directions for future research .
	manualset3
91300	5	399174	13	NULL	NULL	0	NULL	clinical and experimental data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	I guest-edited the present issue of Current Drug Targets aiming to bring together a number of leading experts in the field of cancer chemoprevention , who would systematically review the evidence ; discuss the clinical and experimental data ; highlight new approaches and promising directions for future research .
	manualset3
91301	6	399174	13	NULL	NULL	NULL	NULL	new approaches	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	I guest-edited the present issue of Current Drug Targets aiming to bring together a number of leading experts in the field of cancer chemoprevention , who would systematically review the evidence ; discuss the clinical and experimental data ; highlight new approaches and promising directions for future research .
	manualset3
91302	7	399174	13	NULL	NULL	0	NULL	promising directions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	I guest-edited the present issue of Current Drug Targets aiming to bring together a number of leading experts in the field of cancer chemoprevention , who would systematically review the evidence ; discuss the clinical and experimental data ; highlight new approaches and promising directions for future research .
	manualset3
91303	8	399174	13	NULL	NULL	0	NULL	future research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	I guest-edited the present issue of Current Drug Targets aiming to bring together a number of leading experts in the field of cancer chemoprevention , who would systematically review the evidence ; discuss the clinical and experimental data ; highlight new approaches and promising directions for future research .
	manualset3
91304	1	399175	13	NULL	NULL	0	NULL	legitimacy 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	I am particularly concerned with the legitimacy these justifications have in the eyes of project beneficiaries .
	manualset3
91305	2	399175	13	NULL	NULL	0	NULL	 justifications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	I am particularly concerned with the legitimacy these justifications have in the eyes of project beneficiaries .
	manualset3
91306	3	399175	13	NULL	NULL	0	NULL	eyes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	I am particularly concerned with the legitimacy these justifications have in the eyes of project beneficiaries .
	manualset3
91307	4	399175	13	NULL	NULL	0	NULL	project beneficiaries	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	I am particularly concerned with the legitimacy these justifications have in the eyes of project beneficiaries .
	manualset3
91308	1	399176	13	NULL	NULL	0	NULL	pattern of mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	I examined the pattern of mortality in the Donner Party , a group of emigrants who became trapped with inadequate food stores in the winter snows of the Sierra Nevada mountains in 1846-1847 .
	manualset3
91309	2	399176	13	NULL	NULL	0	NULL	Donner Party	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	I examined the pattern of mortality in the Donner Party , a group of emigrants who became trapped with inadequate food stores in the winter snows of the Sierra Nevada mountains in 1846-1847 .
	manualset3
91310	3	399176	13	NULL	NULL	0	NULL	a group of emigrants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	I examined the pattern of mortality in the Donner Party , a group of emigrants who became trapped with inadequate food stores in the winter snows of the Sierra Nevada mountains in 1846-1847 .
	manualset3
91311	4	399176	13	NULL	NULL	NULL	NULL	food stores	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	I examined the pattern of mortality in the Donner Party , a group of emigrants who became trapped with inadequate food stores in the winter snows of the Sierra Nevada mountains in 1846-1847 .
	manualset3
91312	5	399176	13	NULL	NULL	0	NULL	winter snows	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	I examined the pattern of mortality in the Donner Party , a group of emigrants who became trapped with inadequate food stores in the winter snows of the Sierra Nevada mountains in 1846-1847 .
	manualset3
91313	6	399176	13	NULL	NULL	0	NULL	 Sierra Nevada mountains	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	I examined the pattern of mortality in the Donner Party , a group of emigrants who became trapped with inadequate food stores in the winter snows of the Sierra Nevada mountains in 1846-1847 .
	manualset3
91314	7	399176	13	NULL	NULL	0	NULL	1846-1847	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	I examined the pattern of mortality in the Donner Party , a group of emigrants who became trapped with inadequate food stores in the winter snows of the Sierra Nevada mountains in 1846-1847 .
	manualset3
91315	1	399177	13	NULL	NULL	NULL	NULL	active participant	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	I have been an active participant and eyewitness , and take full responsibility for attempting to write an early history at a time when most of the contributors are still alive .
	manualset3
91316	2	399177	13	NULL	NULL	0	NULL	eyewitness	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	I have been an active participant and eyewitness , and take full responsibility for attempting to write an early history at a time when most of the contributors are still alive .
	manualset3
91317	3	399177	13	NULL	NULL	0	NULL	responsibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	I have been an active participant and eyewitness , and take full responsibility for attempting to write an early history at a time when most of the contributors are still alive .
	manualset3
91318	4	399177	13	NULL	NULL	0	NULL	 time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	I have been an active participant and eyewitness , and take full responsibility for attempting to write an early history at a time when most of the contributors are still alive .
	manualset3
91319	5	399177	13	NULL	NULL	0	NULL	contributors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	I have been an active participant and eyewitness , and take full responsibility for attempting to write an early history at a time when most of the contributors are still alive .
	manualset3
91320	6	399177	13	NULL	NULL	0	NULL	alive	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	I have been an active participant and eyewitness , and take full responsibility for attempting to write an early history at a time when most of the contributors are still alive .
	manualset3
92130	7	399177	13	NULL	NULL	0	NULL	early history	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	I have been an active participant and eyewitness , and take full responsibility for attempting to write an early history at a time when most of the contributors are still alive .
	manualset3
91321	1	399178	13	NULL	NULL	0	NULL	perspectives	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	I hope to provide new perspectives and experimental approaches that go beyond the current state of the art to foster an understanding of eutherian embryogenesis and provide clues for the efficient production of somatic cells for cell therapy .
	manualset3
91322	2	399178	13	NULL	NULL	0	NULL	experimental approaches 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	I hope to provide new perspectives and experimental approaches that go beyond the current state of the art to foster an understanding of eutherian embryogenesis and provide clues for the efficient production of somatic cells for cell therapy .
	manualset3
91323	3	399178	13	NULL	NULL	0	NULL	 current state of the art	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	I hope to provide new perspectives and experimental approaches that go beyond the current state of the art to foster an understanding of eutherian embryogenesis and provide clues for the efficient production of somatic cells for cell therapy .
	manualset3
91324	4	399178	13	NULL	NULL	0	NULL	eutherian embryogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	I hope to provide new perspectives and experimental approaches that go beyond the current state of the art to foster an understanding of eutherian embryogenesis and provide clues for the efficient production of somatic cells for cell therapy .
	manualset3
91325	5	399178	13	NULL	NULL	0	NULL	clues	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	I hope to provide new perspectives and experimental approaches that go beyond the current state of the art to foster an understanding of eutherian embryogenesis and provide clues for the efficient production of somatic cells for cell therapy .
	manualset3
91326	6	399178	13	NULL	NULL	0	NULL	efficient production 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	I hope to provide new perspectives and experimental approaches that go beyond the current state of the art to foster an understanding of eutherian embryogenesis and provide clues for the efficient production of somatic cells for cell therapy .
	manualset3
91327	7	399178	13	NULL	NULL	0	NULL	somatic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	I hope to provide new perspectives and experimental approaches that go beyond the current state of the art to foster an understanding of eutherian embryogenesis and provide clues for the efficient production of somatic cells for cell therapy .
	manualset3
91328	8	399178	13	NULL	NULL	0	NULL	cell therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	I hope to provide new perspectives and experimental approaches that go beyond the current state of the art to foster an understanding of eutherian embryogenesis and provide clues for the efficient production of somatic cells for cell therapy .
	manualset3
91329	1	399179	13	NULL	NULL	0	NULL	Anemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Anemia following partial gastrectomy ) .
	manualset3
91330	2	399179	13	NULL	NULL	0	NULL	 partial gastrectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Anemia following partial gastrectomy ) .
	manualset3
91331	1	399180	13	NULL	NULL	0	NULL	role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( The role of bone marrow stromal cells in apoptosis in myelodysplastic syndrome ) .
	manualset3
91332	2	399180	13	NULL	NULL	0	NULL	bone marrow stromal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	( The role of bone marrow stromal cells in apoptosis in myelodysplastic syndrome ) .
	manualset3
91333	3	399180	13	NULL	NULL	0	NULL	apoptosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( The role of bone marrow stromal cells in apoptosis in myelodysplastic syndrome ) .
	manualset3
91334	4	399180	13	NULL	NULL	0	NULL	myelodysplastic syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( The role of bone marrow stromal cells in apoptosis in myelodysplastic syndrome ) .
	manualset3
91335	1	399181	13	NULL	NULL	0	NULL	emotions	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	I will argue that emotions are constitutively and discursively relevant features of the evaluative experience of persons .
	manualset3
91336	2	399181	13	NULL	NULL	0	NULL	features	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	I will argue that emotions are constitutively and discursively relevant features of the evaluative experience of persons .
	manualset3
91337	3	399181	13	NULL	NULL	NULL	NULL	evaluative experience	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	I will argue that emotions are constitutively and discursively relevant features of the evaluative experience of persons .
	manualset3
91338	4	399181	13	NULL	NULL	0	NULL	persons	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	I will argue that emotions are constitutively and discursively relevant features of the evaluative experience of persons .
	manualset3
91339	1	399182	13	NULL	NULL	NULL	NULL	IAEA/WHO TLD postal dose audit service	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	IAEA/WHO TLD postal dose audit service and high precision measurements for radiotherapy level dosimetry .
	manualset3
91340	2	399182	13	NULL	NULL	0	NULL	precision measurements	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	IAEA/WHO TLD postal dose audit service and high precision measurements for radiotherapy level dosimetry .
	manualset3
91341	3	399182	13	NULL	NULL	0	NULL	radiotherapy level dosimetry	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	IAEA/WHO TLD postal dose audit service and high precision measurements for radiotherapy level dosimetry .
	manualset3
91342	1	399183	13	NULL	NULL	0	NULL	IBD patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	IBD patients may require long-term immunosuppression , and therefore should be considered candidates for vaccination against new HBV infection as well as prophylaxis against HBV reactivation prior to immunosuppressive therapy .
	manualset3
91343	2	399183	13	NULL	NULL	0	NULL	long-term immunosuppression	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	IBD patients may require long-term immunosuppression , and therefore should be considered candidates for vaccination against new HBV infection as well as prophylaxis against HBV reactivation prior to immunosuppressive therapy .
	manualset3
91344	3	399183	13	NULL	NULL	0	NULL	candidates	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	IBD patients may require long-term immunosuppression , and therefore should be considered candidates for vaccination against new HBV infection as well as prophylaxis against HBV reactivation prior to immunosuppressive therapy .
	manualset3
91345	4	399183	13	NULL	NULL	0	NULL	vaccination 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	IBD patients may require long-term immunosuppression , and therefore should be considered candidates for vaccination against new HBV infection as well as prophylaxis against HBV reactivation prior to immunosuppressive therapy .
	manualset3
91346	5	399183	13	NULL	NULL	0	NULL	 HBV infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	IBD patients may require long-term immunosuppression , and therefore should be considered candidates for vaccination against new HBV infection as well as prophylaxis against HBV reactivation prior to immunosuppressive therapy .
	manualset3
91347	6	399183	13	NULL	NULL	0	NULL	prophylaxis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	IBD patients may require long-term immunosuppression , and therefore should be considered candidates for vaccination against new HBV infection as well as prophylaxis against HBV reactivation prior to immunosuppressive therapy .
	manualset3
91348	7	399183	13	NULL	NULL	0	NULL	HBV reactivation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	IBD patients may require long-term immunosuppression , and therefore should be considered candidates for vaccination against new HBV infection as well as prophylaxis against HBV reactivation prior to immunosuppressive therapy .
	manualset3
91349	8	399183	13	NULL	NULL	0	NULL	immunosuppressive therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	IBD patients may require long-term immunosuppression , and therefore should be considered candidates for vaccination against new HBV infection as well as prophylaxis against HBV reactivation prior to immunosuppressive therapy .
	manualset3
91350	1	399184	13	NULL	NULL	0	NULL	ICI 182 780 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	ICI 182 780 did not suppress E2-stimulated IGF-I mRNA expression and 100 nM ICI 182 780 enhanced ( 93 % , p & lt ; 0.05 ) IGF-I mRNA levels in BSC cultures .
	manualset3
91351	2	399184	13	NULL	NULL	0	NULL	E2-stimulated IGF-I mRNA expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	ICI 182 780 did not suppress E2-stimulated IGF-I mRNA expression and 100 nM ICI 182 780 enhanced ( 93 % , p & lt ; 0.05 ) IGF-I mRNA levels in BSC cultures .
	manualset3
91352	3	399184	13	NULL	NULL	0	NULL	100 nM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	ICI 182 780 did not suppress E2-stimulated IGF-I mRNA expression and 100 nM ICI 182 780 enhanced ( 93 % , p & lt ; 0.05 ) IGF-I mRNA levels in BSC cultures .
	manualset3
91353	4	399184	13	NULL	NULL	0	NULL	ICI 182 780	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	ICI 182 780 did not suppress E2-stimulated IGF-I mRNA expression and 100 nM ICI 182 780 enhanced ( 93 % , p & lt ; 0.05 ) IGF-I mRNA levels in BSC cultures .
	manualset3
91354	5	399184	13	NULL	NULL	0	NULL	93 % , p & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	ICI 182 780 did not suppress E2-stimulated IGF-I mRNA expression and 100 nM ICI 182 780 enhanced ( 93 % , p & lt ; 0.05 ) IGF-I mRNA levels in BSC cultures .
	manualset3
91355	6	399184	13	NULL	NULL	0	NULL	 IGF-I mRNA levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	ICI 182 780 did not suppress E2-stimulated IGF-I mRNA expression and 100 nM ICI 182 780 enhanced ( 93 % , p & lt ; 0.05 ) IGF-I mRNA levels in BSC cultures .
	manualset3
91356	7	399184	13	NULL	NULL	0	NULL	BSC cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	ICI 182 780 did not suppress E2-stimulated IGF-I mRNA expression and 100 nM ICI 182 780 enhanced ( 93 % , p & lt ; 0.05 ) IGF-I mRNA levels in BSC cultures .
	manualset3
91357	1	399185	13	NULL	NULL	0	NULL	ICW	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	ICW was similar in both groups but the ICW to ECW ratio was significantly higher in the athletes compared to the recreational sportsmen ( 0.67 + / - 0.16 vs 0.54 + / - 0.07 , p & lt ; 0.01 ) .
	manualset3
91358	2	399185	13	NULL	NULL	0	NULL	both groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	ICW was similar in both groups but the ICW to ECW ratio was significantly higher in the athletes compared to the recreational sportsmen ( 0.67 + / - 0.16 vs 0.54 + / - 0.07 , p & lt ; 0.01 ) .
	manualset3
91359	3	399185	13	NULL	NULL	0	NULL	ICW to ECW ratio	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	ICW was similar in both groups but the ICW to ECW ratio was significantly higher in the athletes compared to the recreational sportsmen ( 0.67 + / - 0.16 vs 0.54 + / - 0.07 , p & lt ; 0.01 ) .
	manualset3
91360	4	399185	13	NULL	NULL	0	NULL	athletes 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	ICW was similar in both groups but the ICW to ECW ratio was significantly higher in the athletes compared to the recreational sportsmen ( 0.67 + / - 0.16 vs 0.54 + / - 0.07 , p & lt ; 0.01 ) .
	manualset3
91361	5	399185	13	NULL	NULL	0	NULL	recreational sportsmen	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	ICW was similar in both groups but the ICW to ECW ratio was significantly higher in the athletes compared to the recreational sportsmen ( 0.67 + / - 0.16 vs 0.54 + / - 0.07 , p & lt ; 0.01 ) .
	manualset3
91362	6	399185	13	NULL	NULL	0	NULL	0.67 + / - 0.16 vs 0.54 + / - 0.07 , p & lt ; 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	ICW was similar in both groups but the ICW to ECW ratio was significantly higher in the athletes compared to the recreational sportsmen ( 0.67 + / - 0.16 vs 0.54 + / - 0.07 , p & lt ; 0.01 ) .
	manualset3
91363	1	399186	13	NULL	NULL	0	NULL	IFN	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IFN arrests the growth of Burkitt Lymphoma derived cell line Daudi cells in the G1 phase .
	manualset3
91364	2	399186	13	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IFN arrests the growth of Burkitt Lymphoma derived cell line Daudi cells in the G1 phase .
	manualset3
91365	3	399186	13	NULL	NULL	0	NULL	Burkitt Lymphoma derived cell line Daudi cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	IFN arrests the growth of Burkitt Lymphoma derived cell line Daudi cells in the G1 phase .
	manualset3
91366	4	399186	13	NULL	NULL	0	NULL	G1 phase	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IFN arrests the growth of Burkitt Lymphoma derived cell line Daudi cells in the G1 phase .
	manualset3
91367	1	399187	13	NULL	NULL	0	NULL	IGF-II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IGF-II was more effective than IGF-I in competitively displacing both labeled ligands .
	manualset3
91368	2	399187	13	NULL	NULL	0	NULL	IGF-I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IGF-II was more effective than IGF-I in competitively displacing both labeled ligands .
	manualset3
91369	3	399187	13	NULL	NULL	0	NULL	labeled ligands	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	IGF-II was more effective than IGF-I in competitively displacing both labeled ligands .
	manualset3
91370	1	399188	13	NULL	NULL	0	NULL	 role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The role of the general practitioner in the control of cancer ) .
	manualset3
91371	2	399188	13	NULL	NULL	0	NULL	general practitioner	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( The role of the general practitioner in the control of cancer ) .
	manualset3
91372	3	399188	13	NULL	NULL	0	NULL	cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( The role of the general practitioner in the control of cancer ) .
	manualset3
91373	1	399189	13	NULL	NULL	0	NULL	IGFBP-2 mRNA levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-2 mRNA levels remained high at the contusion site in the presence of either drug , but the increase was blocked in the cortex temporal to the impact by MK-801 .
	manualset3
91374	2	399189	13	NULL	NULL	0	NULL	 contusion site	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-2 mRNA levels remained high at the contusion site in the presence of either drug , but the increase was blocked in the cortex temporal to the impact by MK-801 .
	manualset3
91375	3	399189	13	NULL	NULL	0	NULL	drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-2 mRNA levels remained high at the contusion site in the presence of either drug , but the increase was blocked in the cortex temporal to the impact by MK-801 .
	manualset3
91376	4	399189	13	NULL	NULL	0	NULL	cortex temporal	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-2 mRNA levels remained high at the contusion site in the presence of either drug , but the increase was blocked in the cortex temporal to the impact by MK-801 .
	manualset3
91377	5	399189	13	NULL	NULL	0	NULL	 impact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-2 mRNA levels remained high at the contusion site in the presence of either drug , but the increase was blocked in the cortex temporal to the impact by MK-801 .
	manualset3
91378	6	399189	13	NULL	NULL	0	NULL	MK-801	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-2 mRNA levels remained high at the contusion site in the presence of either drug , but the increase was blocked in the cortex temporal to the impact by MK-801 .
	manualset3
91379	7	399189	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	IGFBP-2 mRNA levels remained high at the contusion site in the presence of either drug , but the increase was blocked in the cortex temporal to the impact by MK-801 .
	manualset3
91380	1	399190	13	NULL	NULL	0	NULL	IGFs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	IGFs are important positive modulators of overall body and muscle growth in different species .
	manualset3
91381	2	399190	13	NULL	NULL	0	NULL	positive modulators	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	IGFs are important positive modulators of overall body and muscle growth in different species .
	manualset3
91382	3	399190	13	NULL	NULL	0	NULL	 overall body	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	IGFs are important positive modulators of overall body and muscle growth in different species .
	manualset3
91383	4	399190	13	NULL	NULL	0	NULL	muscle growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IGFs are important positive modulators of overall body and muscle growth in different species .
	manualset3
91384	5	399190	13	NULL	NULL	0	NULL	species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	IGFs are important positive modulators of overall body and muscle growth in different species .
	manualset3
91385	1	399191	13	NULL	NULL	0	NULL	IHD	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	IHD correlated with SA ( r = 0.25-0 .27 , p = 0.006-0 .0026 ) , only in the 74 year age group .
	manualset3
91386	2	399191	13	NULL	NULL	0	NULL	SA ( r = 0.25-0 .27 , p = 0.006-0 .0026 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	IHD correlated with SA ( r = 0.25-0 .27 , p = 0.006-0 .0026 ) , only in the 74 year age group .
	manualset3
91387	3	399191	13	NULL	NULL	0	NULL	74 year age group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	IHD correlated with SA ( r = 0.25-0 .27 , p = 0.006-0 .0026 ) , only in the 74 year age group .
	manualset3
91388	1	399192	13	NULL	NULL	0	NULL	RIAMAT T4 kit	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	II : RIAMAT T4 kit ( author 's transl ) ) .
	manualset3
91389	2	399192	13	NULL	NULL	0	NULL	author 's	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	II : RIAMAT T4 kit ( author 's transl ) ) .
	manualset3
91390	1	399193	13	NULL	NULL	0	NULL	IISs	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	IISs propagate to L2/3 via activation of L2/3 interneurons but not pyramidal cells , which are mostly quiescent at this phase .
	manualset3
91391	2	399193	13	NULL	NULL	0	NULL	L2/3	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	IISs propagate to L2/3 via activation of L2/3 interneurons but not pyramidal cells , which are mostly quiescent at this phase .
	manualset3
91392	3	399193	13	NULL	NULL	0	NULL	 activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IISs propagate to L2/3 via activation of L2/3 interneurons but not pyramidal cells , which are mostly quiescent at this phase .
	manualset3
91393	4	399193	13	NULL	NULL	0	NULL	L2/3 interneurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	IISs propagate to L2/3 via activation of L2/3 interneurons but not pyramidal cells , which are mostly quiescent at this phase .
	manualset3
91394	5	399193	13	NULL	NULL	0	NULL	 pyramidal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	IISs propagate to L2/3 via activation of L2/3 interneurons but not pyramidal cells , which are mostly quiescent at this phase .
	manualset3
91395	6	399193	13	NULL	NULL	0	NULL	phase	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IISs propagate to L2/3 via activation of L2/3 interneurons but not pyramidal cells , which are mostly quiescent at this phase .
	manualset3
91396	1	399194	13	NULL	NULL	NULL	NULL	IK	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	IK , IR recorded in GH3/B6 cells and ERG currents in CHO cells were compared using similar experimental conditions ( same pulse protocols and isotonic KCl as extracellular solution ) .
	manualset3
91397	2	399194	13	NULL	NULL	0	NULL	IR 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	IK , IR recorded in GH3/B6 cells and ERG currents in CHO cells were compared using similar experimental conditions ( same pulse protocols and isotonic KCl as extracellular solution ) .
	manualset3
91398	3	399194	13	NULL	NULL	0	NULL	GH3/B6 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	IK , IR recorded in GH3/B6 cells and ERG currents in CHO cells were compared using similar experimental conditions ( same pulse protocols and isotonic KCl as extracellular solution ) .
	manualset3
91399	4	399194	13	NULL	NULL	0	NULL	ERG currents 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	IK , IR recorded in GH3/B6 cells and ERG currents in CHO cells were compared using similar experimental conditions ( same pulse protocols and isotonic KCl as extracellular solution ) .
	manualset3
91400	5	399194	13	NULL	NULL	0	NULL	 CHO cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	IK , IR recorded in GH3/B6 cells and ERG currents in CHO cells were compared using similar experimental conditions ( same pulse protocols and isotonic KCl as extracellular solution ) .
	manualset3
91401	6	399194	13	NULL	NULL	0	NULL	experimental conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	IK , IR recorded in GH3/B6 cells and ERG currents in CHO cells were compared using similar experimental conditions ( same pulse protocols and isotonic KCl as extracellular solution ) .
	manualset3
91402	7	399194	13	NULL	NULL	0	NULL	pulse protocols	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	IK , IR recorded in GH3/B6 cells and ERG currents in CHO cells were compared using similar experimental conditions ( same pulse protocols and isotonic KCl as extracellular solution ) .
	manualset3
91403	8	399194	13	NULL	NULL	0	NULL	isotonic KCl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	IK , IR recorded in GH3/B6 cells and ERG currents in CHO cells were compared using similar experimental conditions ( same pulse protocols and isotonic KCl as extracellular solution ) .
	manualset3
91404	9	399194	13	NULL	NULL	0	NULL	extracellular solution 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	IK , IR recorded in GH3/B6 cells and ERG currents in CHO cells were compared using similar experimental conditions ( same pulse protocols and isotonic KCl as extracellular solution ) .
	manualset3
91405	1	399195	13	NULL	NULL	0	NULL	IK2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IK2 inhibits development of malaria sporozoites present in the mosquito salivary glands .
	manualset3
91406	2	399195	13	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IK2 inhibits development of malaria sporozoites present in the mosquito salivary glands .
	manualset3
91407	3	399195	13	NULL	NULL	0	NULL	malaria sporozoites 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	IK2 inhibits development of malaria sporozoites present in the mosquito salivary glands .
	manualset3
91408	4	399195	13	NULL	NULL	0	NULL	mosquito salivary glands 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	IK2 inhibits development of malaria sporozoites present in the mosquito salivary glands .
	manualset3
91409	1	399196	13	NULL	NULL	0	NULL	IL-1 / IL-1 receptor complex signaling 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-1 / IL-1 receptor complex signaling requires adaptor proteins , e.g. , the IL-1 receptor brain-specific accessory protein ( AcPb ) .
	manualset3
91410	2	399196	13	NULL	NULL	0	NULL	adaptor proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-1 / IL-1 receptor complex signaling requires adaptor proteins , e.g. , the IL-1 receptor brain-specific accessory protein ( AcPb ) .
	manualset3
91411	3	399196	13	NULL	NULL	0	NULL	IL-1 receptor brain-specific accessory protein ( AcPb ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-1 / IL-1 receptor complex signaling requires adaptor proteins , e.g. , the IL-1 receptor brain-specific accessory protein ( AcPb ) .
	manualset3
91412	1	399197	13	NULL	NULL	0	NULL	 role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The role of the pharmacist in the management of the operating room ) .
	manualset3
91413	2	399197	13	NULL	NULL	0	NULL	pharmacist	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( The role of the pharmacist in the management of the operating room ) .
	manualset3
91414	3	399197	13	NULL	NULL	0	NULL	management 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The role of the pharmacist in the management of the operating room ) .
	manualset3
91415	4	399197	13	NULL	NULL	0	NULL	operating room 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( The role of the pharmacist in the management of the operating room ) .
	manualset3
91416	1	399198	13	NULL	NULL	0	NULL	IL-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-1 activation of NF-B was inhibited by NPY treatment , as observed by confocal microscopy and Western blotting analysis of nuclear translocation of NF-B p65 subunit , leading to the decrease of NO synthesis .
	manualset3
91417	2	399198	13	NULL	NULL	0	NULL	 activation of NF-B	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-1 activation of NF-B was inhibited by NPY treatment , as observed by confocal microscopy and Western blotting analysis of nuclear translocation of NF-B p65 subunit , leading to the decrease of NO synthesis .
	manualset3
91418	3	399198	13	NULL	NULL	0	NULL	NPY	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-1 activation of NF-B was inhibited by NPY treatment , as observed by confocal microscopy and Western blotting analysis of nuclear translocation of NF-B p65 subunit , leading to the decrease of NO synthesis .
	manualset3
91419	4	399198	13	NULL	NULL	0	NULL	 treatment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-1 activation of NF-B was inhibited by NPY treatment , as observed by confocal microscopy and Western blotting analysis of nuclear translocation of NF-B p65 subunit , leading to the decrease of NO synthesis .
	manualset3
91420	5	399198	13	NULL	NULL	0	NULL	 confocal microscopy 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-1 activation of NF-B was inhibited by NPY treatment , as observed by confocal microscopy and Western blotting analysis of nuclear translocation of NF-B p65 subunit , leading to the decrease of NO synthesis .
	manualset3
91421	6	399198	13	NULL	NULL	0	NULL	Western blotting analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-1 activation of NF-B was inhibited by NPY treatment , as observed by confocal microscopy and Western blotting analysis of nuclear translocation of NF-B p65 subunit , leading to the decrease of NO synthesis .
	manualset3
91422	7	399198	13	NULL	NULL	0	NULL	 nuclear translocation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-1 activation of NF-B was inhibited by NPY treatment , as observed by confocal microscopy and Western blotting analysis of nuclear translocation of NF-B p65 subunit , leading to the decrease of NO synthesis .
	manualset3
91423	8	399198	13	NULL	NULL	0	NULL	NF-B p65 subunit 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-1 activation of NF-B was inhibited by NPY treatment , as observed by confocal microscopy and Western blotting analysis of nuclear translocation of NF-B p65 subunit , leading to the decrease of NO synthesis .
	manualset3
91424	9	399198	13	NULL	NULL	0	NULL	decrease of NO synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-1 activation of NF-B was inhibited by NPY treatment , as observed by confocal microscopy and Western blotting analysis of nuclear translocation of NF-B p65 subunit , leading to the decrease of NO synthesis .
	manualset3
91425	1	399199	13	NULL	NULL	0	NULL	IL-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-1 and TNF-alpha induced mRNA expression of c-jun while IL-17 had no effect .
	manualset3
91426	2	399199	13	NULL	NULL	0	NULL	TNF-alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-1 and TNF-alpha induced mRNA expression of c-jun while IL-17 had no effect .
	manualset3
91427	3	399199	13	NULL	NULL	0	NULL	mRNA expression of c-jun	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-1 and TNF-alpha induced mRNA expression of c-jun while IL-17 had no effect .
	manualset3
91428	4	399199	13	NULL	NULL	0	NULL	IL-17	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-1 and TNF-alpha induced mRNA expression of c-jun while IL-17 had no effect .
	manualset3
91429	1	399200	13	NULL	NULL	0	NULL	IL-1 beta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-1 beta is secreted by activated murine macrophages as biologically inactive precursor .
	manualset3
91430	2	399200	13	NULL	NULL	0	NULL	murine macrophages 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-1 beta is secreted by activated murine macrophages as biologically inactive precursor .
	manualset3
91431	3	399200	13	NULL	NULL	0	NULL	biologically inactive precursor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-1 beta is secreted by activated murine macrophages as biologically inactive precursor .
	manualset3
91432	1	399201	13	NULL	NULL	NULL	NULL	IL-1	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	IL-1 is a pro-inflammatory cytokine consisted of two molecular species , IL-1alpha and IL-1beta , and the IL-1 receptor antagonist ( IL-1Ra ) is a natural inhibitor of both molecules .
	manualset3
91433	2	399201	13	NULL	NULL	NULL	NULL	pro-inflammatory cytokine	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	IL-1 is a pro-inflammatory cytokine consisted of two molecular species , IL-1alpha and IL-1beta , and the IL-1 receptor antagonist ( IL-1Ra ) is a natural inhibitor of both molecules .
	manualset3
91434	3	399201	13	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-1 is a pro-inflammatory cytokine consisted of two molecular species , IL-1alpha and IL-1beta , and the IL-1 receptor antagonist ( IL-1Ra ) is a natural inhibitor of both molecules .
	manualset3
91435	4	399201	13	NULL	NULL	0	NULL	molecular species 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-1 is a pro-inflammatory cytokine consisted of two molecular species , IL-1alpha and IL-1beta , and the IL-1 receptor antagonist ( IL-1Ra ) is a natural inhibitor of both molecules .
	manualset3
91436	5	399201	13	NULL	NULL	0	NULL	IL-1alpha 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-1 is a pro-inflammatory cytokine consisted of two molecular species , IL-1alpha and IL-1beta , and the IL-1 receptor antagonist ( IL-1Ra ) is a natural inhibitor of both molecules .
	manualset3
91437	6	399201	13	NULL	NULL	0	NULL	IL-1beta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-1 is a pro-inflammatory cytokine consisted of two molecular species , IL-1alpha and IL-1beta , and the IL-1 receptor antagonist ( IL-1Ra ) is a natural inhibitor of both molecules .
	manualset3
91438	7	399201	13	NULL	NULL	0	NULL	IL-1 receptor antagonist ( IL-1Ra )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-1 is a pro-inflammatory cytokine consisted of two molecular species , IL-1alpha and IL-1beta , and the IL-1 receptor antagonist ( IL-1Ra ) is a natural inhibitor of both molecules .
	manualset3
91439	8	399201	13	NULL	NULL	0	NULL	natural inhibitor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-1 is a pro-inflammatory cytokine consisted of two molecular species , IL-1alpha and IL-1beta , and the IL-1 receptor antagonist ( IL-1Ra ) is a natural inhibitor of both molecules .
	manualset3
91440	9	399201	13	NULL	NULL	0	NULL	molecules	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-1 is a pro-inflammatory cytokine consisted of two molecular species , IL-1alpha and IL-1beta , and the IL-1 receptor antagonist ( IL-1Ra ) is a natural inhibitor of both molecules .
	manualset3
91441	1	399202	13	NULL	NULL	0	NULL	IL-12 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-12 protects against coxsackievirus B3-induced myocarditis by increasing IFN-gamma and macrophage and neutrophil populations in the heart .
	manualset3
91442	2	399202	13	NULL	NULL	0	NULL	coxsackievirus B3-induced myocarditis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-12 protects against coxsackievirus B3-induced myocarditis by increasing IFN-gamma and macrophage and neutrophil populations in the heart .
	manualset3
91443	3	399202	13	NULL	NULL	0	NULL	IFN-gamma 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-12 protects against coxsackievirus B3-induced myocarditis by increasing IFN-gamma and macrophage and neutrophil populations in the heart .
	manualset3
91444	4	399202	13	NULL	NULL	0	NULL	macrophage populations	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-12 protects against coxsackievirus B3-induced myocarditis by increasing IFN-gamma and macrophage and neutrophil populations in the heart .
	manualset3
91445	5	399202	13	NULL	NULL	0	NULL	neutrophil populations	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-12 protects against coxsackievirus B3-induced myocarditis by increasing IFN-gamma and macrophage and neutrophil populations in the heart .
	manualset3
91446	6	399202	13	NULL	NULL	0	NULL	heart	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-12 protects against coxsackievirus B3-induced myocarditis by increasing IFN-gamma and macrophage and neutrophil populations in the heart .
	manualset3
91447	1	399203	13	NULL	NULL	0	NULL	IL-13	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-13 induces mucin production by stimulating epidermal growth factor receptors and by activating neutrophils .
	manualset3
91448	2	399203	13	NULL	NULL	0	NULL	mucin production 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-13 induces mucin production by stimulating epidermal growth factor receptors and by activating neutrophils .
	manualset3
91449	3	399203	13	NULL	NULL	0	NULL	epidermal growth factor receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-13 induces mucin production by stimulating epidermal growth factor receptors and by activating neutrophils .
	manualset3
91450	4	399203	13	NULL	NULL	0	NULL	neutrophils	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-13 induces mucin production by stimulating epidermal growth factor receptors and by activating neutrophils .
	manualset3
91451	1	399204	13	NULL	NULL	0	NULL	IL-17 expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-17 expression by mycobacteria-specific disease site T cells was not detected in healthy , M.tb-infected persons , or patients with TB pericarditis .
	manualset3
91452	2	399204	13	NULL	NULL	0	NULL	mycobacteria-specific disease site T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-17 expression by mycobacteria-specific disease site T cells was not detected in healthy , M.tb-infected persons , or patients with TB pericarditis .
	manualset3
91453	3	399204	13	NULL	NULL	0	NULL	healthy persons	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-17 expression by mycobacteria-specific disease site T cells was not detected in healthy , M.tb-infected persons , or patients with TB pericarditis .
	manualset3
91454	4	399204	13	NULL	NULL	0	NULL	M.tb-infected persons	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-17 expression by mycobacteria-specific disease site T cells was not detected in healthy , M.tb-infected persons , or patients with TB pericarditis .
	manualset3
91455	5	399204	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-17 expression by mycobacteria-specific disease site T cells was not detected in healthy , M.tb-infected persons , or patients with TB pericarditis .
	manualset3
91456	6	399204	13	NULL	NULL	0	NULL	TB pericarditis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-17 expression by mycobacteria-specific disease site T cells was not detected in healthy , M.tb-infected persons , or patients with TB pericarditis .
	manualset3
91457	1	399205	13	NULL	NULL	0	NULL	IL-18	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-18 produced by DCs and macrophages acts in an autocrine manner and augments IL-12-induced IFN-gamma production by DCs as also observed in T and NK cells .
	manualset3
91458	2	399205	13	NULL	NULL	0	NULL	DCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-18 produced by DCs and macrophages acts in an autocrine manner and augments IL-12-induced IFN-gamma production by DCs as also observed in T and NK cells .
	manualset3
91459	3	399205	13	NULL	NULL	0	NULL	macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-18 produced by DCs and macrophages acts in an autocrine manner and augments IL-12-induced IFN-gamma production by DCs as also observed in T and NK cells .
	manualset3
91461	5	399205	13	NULL	NULL	0	NULL	autocrine manner 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-18 produced by DCs and macrophages acts in an autocrine manner and augments IL-12-induced IFN-gamma production by DCs as also observed in T and NK cells .
	manualset3
91462	6	399205	13	NULL	NULL	0	NULL	IL-12-induced IFN-gamma production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-18 produced by DCs and macrophages acts in an autocrine manner and augments IL-12-induced IFN-gamma production by DCs as also observed in T and NK cells .
	manualset3
91463	7	399205	13	NULL	NULL	0	NULL	DCs 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-18 produced by DCs and macrophages acts in an autocrine manner and augments IL-12-induced IFN-gamma production by DCs as also observed in T and NK cells .
	manualset3
91464	8	399205	13	NULL	NULL	0	NULL	T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-18 produced by DCs and macrophages acts in an autocrine manner and augments IL-12-induced IFN-gamma production by DCs as also observed in T and NK cells .
	manualset3
91465	9	399205	13	NULL	NULL	0	NULL	NK cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-18 produced by DCs and macrophages acts in an autocrine manner and augments IL-12-induced IFN-gamma production by DCs as also observed in T and NK cells .
	manualset3
91466	1	399206	13	NULL	NULL	0	NULL	IL-2-dependent T effector cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-2-dependent T effector cells usually die when deprived of growth factor .
	manualset3
91467	2	399206	13	NULL	NULL	0	NULL	growth factor	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-2-dependent T effector cells usually die when deprived of growth factor .
	manualset3
91468	1	399207	13	NULL	NULL	0	NULL	small RNAs 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	( The small RNAs in plant immunity ) .
	manualset3
91469	2	399207	13	NULL	NULL	0	NULL	plant	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( The small RNAs in plant immunity ) .
	manualset3
91470	3	399207	13	NULL	NULL	0	NULL	immunity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( The small RNAs in plant immunity ) .
	manualset3
91471	1	399208	13	NULL	NULL	0	NULL	IL-2 levels 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-2 , IL-10 , TNF-alpha , C3 , and C4 levels were significantly elevated in the patient group .
	manualset3
91472	2	399208	13	NULL	NULL	0	NULL	IL-10 levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-2 , IL-10 , TNF-alpha , C3 , and C4 levels were significantly elevated in the patient group .
	manualset3
91473	3	399208	13	NULL	NULL	0	NULL	TNF-alpha levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-2 , IL-10 , TNF-alpha , C3 , and C4 levels were significantly elevated in the patient group .
	manualset3
91474	4	399208	13	NULL	NULL	0	NULL	C3 levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-2 , IL-10 , TNF-alpha , C3 , and C4 levels were significantly elevated in the patient group .
	manualset3
92438	5	399208	13	NULL	NULL	0	NULL	patient group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-2 , IL-10 , TNF-alpha , C3 , and C4 levels were significantly elevated in the patient group .
	manualset3
91475	1	399209	13	NULL	NULL	0	NULL	IL-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-2 and IL-4 stimulated the expression of MEK1 and c-Fos and induced T cell resistance .
	manualset3
91476	2	399209	13	NULL	NULL	0	NULL	IL-4 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-2 and IL-4 stimulated the expression of MEK1 and c-Fos and induced T cell resistance .
	manualset3
91477	3	399209	13	NULL	NULL	0	NULL	expression of MEK1	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-2 and IL-4 stimulated the expression of MEK1 and c-Fos and induced T cell resistance .
	manualset3
91478	4	399209	13	NULL	NULL	0	NULL	expression of c-Fos	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-2 and IL-4 stimulated the expression of MEK1 and c-Fos and induced T cell resistance .
	manualset3
91479	5	399209	13	NULL	NULL	0	NULL	T cell resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-2 and IL-4 stimulated the expression of MEK1 and c-Fos and induced T cell resistance .
	manualset3
91480	1	399210	13	NULL	NULL	0	NULL	IL-27 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-27 regulates IL-12 responsiveness of naive CD4 + T cells through Stat1-dependent and - independent mechanisms .
	manualset3
91481	2	399210	13	NULL	NULL	0	NULL	IL-12 responsiveness	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-27 regulates IL-12 responsiveness of naive CD4 + T cells through Stat1-dependent and - independent mechanisms .
	manualset3
91482	3	399210	13	NULL	NULL	0	NULL	naive CD4 + T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-27 regulates IL-12 responsiveness of naive CD4 + T cells through Stat1-dependent and - independent mechanisms .
	manualset3
91483	4	399210	13	NULL	NULL	0	NULL	 Stat1-dependent mechanisms 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-27 regulates IL-12 responsiveness of naive CD4 + T cells through Stat1-dependent and - independent mechanisms .
	manualset3
91484	5	399210	13	NULL	NULL	0	NULL	Stat1- independent mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-27 regulates IL-12 responsiveness of naive CD4 + T cells through Stat1-dependent and - independent mechanisms .
	manualset3
91485	1	399211	13	NULL	NULL	0	NULL	IL-4 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-4 and interferon-gamma production in children with atopic disease .
	manualset3
91486	2	399211	13	NULL	NULL	0	NULL	interferon-gamma	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-4 and interferon-gamma production in children with atopic disease .
	manualset3
91487	3	399211	13	NULL	NULL	0	NULL	production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-4 and interferon-gamma production in children with atopic disease .
	manualset3
91488	4	399211	13	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-4 and interferon-gamma production in children with atopic disease .
	manualset3
91489	5	399211	13	NULL	NULL	0	NULL	 atopic disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-4 and interferon-gamma production in children with atopic disease .
	manualset3
91490	1	399212	13	NULL	NULL	0	NULL	IL-4 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-4 inhibited the spontaneous proliferation found in three cases , but stimulated proliferation after CD40 crosslinking .
	manualset3
91491	2	399212	13	NULL	NULL	0	NULL	spontaneous proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-4 inhibited the spontaneous proliferation found in three cases , but stimulated proliferation after CD40 crosslinking .
	manualset3
91492	3	399212	13	NULL	NULL	0	NULL	three cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-4 inhibited the spontaneous proliferation found in three cases , but stimulated proliferation after CD40 crosslinking .
	manualset3
91493	4	399212	13	NULL	NULL	0	NULL	proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-4 inhibited the spontaneous proliferation found in three cases , but stimulated proliferation after CD40 crosslinking .
	manualset3
91494	5	399212	13	NULL	NULL	0	NULL	CD40 crosslinking 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-4 inhibited the spontaneous proliferation found in three cases , but stimulated proliferation after CD40 crosslinking .
	manualset3
91495	1	399213	13	NULL	NULL	0	NULL	IL-5-producing T cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-5-producing T cells that induce airway eosinophilia and hyperresponsiveness are suppressed by dexamethasone and cyclosporin A in mice .
	manualset3
91496	2	399213	13	NULL	NULL	0	NULL	airway eosinophilia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-5-producing T cells that induce airway eosinophilia and hyperresponsiveness are suppressed by dexamethasone and cyclosporin A in mice .
	manualset3
91497	3	399213	13	NULL	NULL	0	NULL	hyperresponsiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-5-producing T cells that induce airway eosinophilia and hyperresponsiveness are suppressed by dexamethasone and cyclosporin A in mice .
	manualset3
91498	4	399213	13	NULL	NULL	0	NULL	dexamethasone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-5-producing T cells that induce airway eosinophilia and hyperresponsiveness are suppressed by dexamethasone and cyclosporin A in mice .
	manualset3
91499	5	399213	13	NULL	NULL	0	NULL	cyclosporin A	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-5-producing T cells that induce airway eosinophilia and hyperresponsiveness are suppressed by dexamethasone and cyclosporin A in mice .
	manualset3
91500	6	399213	13	NULL	NULL	0	NULL	 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-5-producing T cells that induce airway eosinophilia and hyperresponsiveness are suppressed by dexamethasone and cyclosporin A in mice .
	manualset3
91501	1	399214	13	NULL	NULL	0	NULL	IL-5 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-5 and IL-13 mRNA were increased in lung tissue of OA-challenged Dcn ( + / + ) mice .
	manualset3
91502	2	399214	13	NULL	NULL	0	NULL	IL-13 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-5 and IL-13 mRNA were increased in lung tissue of OA-challenged Dcn ( + / + ) mice .
	manualset3
91503	3	399214	13	NULL	NULL	0	NULL	lung tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-5 and IL-13 mRNA were increased in lung tissue of OA-challenged Dcn ( + / + ) mice .
	manualset3
91504	4	399214	13	NULL	NULL	0	NULL	OA-challenged Dcn ( + / + ) mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-5 and IL-13 mRNA were increased in lung tissue of OA-challenged Dcn ( + / + ) mice .
	manualset3
91505	1	399215	13	NULL	NULL	0	NULL	IL-5 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-5 is produced by both hematopoietic and non-hematopoietic cells including T cells , granulocytes , and natural helper cells .
	manualset3
91506	2	399215	13	NULL	NULL	0	NULL	hematopoietic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-5 is produced by both hematopoietic and non-hematopoietic cells including T cells , granulocytes , and natural helper cells .
	manualset3
91507	3	399215	13	NULL	NULL	0	NULL	non-hematopoietic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-5 is produced by both hematopoietic and non-hematopoietic cells including T cells , granulocytes , and natural helper cells .
	manualset3
91508	4	399215	13	NULL	NULL	0	NULL	T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-5 is produced by both hematopoietic and non-hematopoietic cells including T cells , granulocytes , and natural helper cells .
	manualset3
91509	5	399215	13	NULL	NULL	0	NULL	granulocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-5 is produced by both hematopoietic and non-hematopoietic cells including T cells , granulocytes , and natural helper cells .
	manualset3
91510	6	399215	13	NULL	NULL	0	NULL	natural helper cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-5 is produced by both hematopoietic and non-hematopoietic cells including T cells , granulocytes , and natural helper cells .
	manualset3
91511	1	399216	13	NULL	NULL	0	NULL	IL-6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-6 also activated the MAPK signaling pathway in adipocytes through the association with its receptor .
	manualset3
91512	2	399216	13	NULL	NULL	0	NULL	MAPK signaling pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-6 also activated the MAPK signaling pathway in adipocytes through the association with its receptor .
	manualset3
91513	3	399216	13	NULL	NULL	0	NULL	adipocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-6 also activated the MAPK signaling pathway in adipocytes through the association with its receptor .
	manualset3
91514	4	399216	13	NULL	NULL	0	NULL	association	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-6 also activated the MAPK signaling pathway in adipocytes through the association with its receptor .
	manualset3
91515	5	399216	13	NULL	NULL	0	NULL	receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-6 also activated the MAPK signaling pathway in adipocytes through the association with its receptor .
	manualset3
91516	1	399217	13	NULL	NULL	0	NULL	state	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The state of the field of hygiene in medicine .
	manualset3
91517	2	399217	13	NULL	NULL	0	NULL	field of hygiene	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( The state of the field of hygiene in medicine .
	manualset3
91518	3	399217	13	NULL	NULL	0	NULL	medicine	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( The state of the field of hygiene in medicine .
	manualset3
91519	1	399218	13	NULL	NULL	0	NULL	IL-6 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-6 or TNF also significantly reduced plasma membrane-associated caveolin-1 .
	manualset3
91520	2	399218	13	NULL	NULL	0	NULL	TNF 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-6 or TNF also significantly reduced plasma membrane-associated caveolin-1 .
	manualset3
91521	3	399218	13	NULL	NULL	0	NULL	plasma membrane-associated caveolin-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-6 or TNF also significantly reduced plasma membrane-associated caveolin-1 .
	manualset3
91522	1	399219	13	NULL	NULL	0	NULL	IL-6 production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-6 production in response to size-fractioned PM exposures failed to show evidence of relative importance of particle sizes in their abilities to induce proinflammatory responses .
	manualset3
91523	2	399219	13	NULL	NULL	0	NULL	response 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-6 production in response to size-fractioned PM exposures failed to show evidence of relative importance of particle sizes in their abilities to induce proinflammatory responses .
	manualset3
91524	3	399219	13	NULL	NULL	0	NULL	size-fractioned PM exposures	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-6 production in response to size-fractioned PM exposures failed to show evidence of relative importance of particle sizes in their abilities to induce proinflammatory responses .
	manualset3
91525	4	399219	13	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-6 production in response to size-fractioned PM exposures failed to show evidence of relative importance of particle sizes in their abilities to induce proinflammatory responses .
	manualset3
91526	5	399219	13	NULL	NULL	0	NULL	relative importance	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-6 production in response to size-fractioned PM exposures failed to show evidence of relative importance of particle sizes in their abilities to induce proinflammatory responses .
	manualset3
91527	6	399219	13	NULL	NULL	0	NULL	particle sizes	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-6 production in response to size-fractioned PM exposures failed to show evidence of relative importance of particle sizes in their abilities to induce proinflammatory responses .
	manualset3
91528	7	399219	13	NULL	NULL	0	NULL	abilities 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-6 production in response to size-fractioned PM exposures failed to show evidence of relative importance of particle sizes in their abilities to induce proinflammatory responses .
	manualset3
91529	8	399219	13	NULL	NULL	0	NULL	proinflammatory responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IL-6 production in response to size-fractioned PM exposures failed to show evidence of relative importance of particle sizes in their abilities to induce proinflammatory responses .
	manualset3
91530	1	399220	13	NULL	NULL	0	NULL	IL 1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IL 1 in combination with ionomycin ( iono/rIL 1 ) stimulated a proliferative response that was associated with the production of IL 4 as measured by lymphokine bioassay and mRNA studies .
	manualset3
91531	2	399220	13	NULL	NULL	0	NULL	ionomycin	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	IL 1 in combination with ionomycin ( iono/rIL 1 ) stimulated a proliferative response that was associated with the production of IL 4 as measured by lymphokine bioassay and mRNA studies .
	manualset3
91532	3	399220	13	NULL	NULL	0	NULL	iono/rIL 1	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	IL 1 in combination with ionomycin ( iono/rIL 1 ) stimulated a proliferative response that was associated with the production of IL 4 as measured by lymphokine bioassay and mRNA studies .
	manualset3
91533	4	399220	13	NULL	NULL	NULL	NULL	proliferative response	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	IL 1 in combination with ionomycin ( iono/rIL 1 ) stimulated a proliferative response that was associated with the production of IL 4 as measured by lymphokine bioassay and mRNA studies .
	manualset3
91534	5	399220	13	NULL	NULL	0	NULL	production of IL 4	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IL 1 in combination with ionomycin ( iono/rIL 1 ) stimulated a proliferative response that was associated with the production of IL 4 as measured by lymphokine bioassay and mRNA studies .
	manualset3
91535	6	399220	13	NULL	NULL	0	NULL	 lymphokine bioassay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	IL 1 in combination with ionomycin ( iono/rIL 1 ) stimulated a proliferative response that was associated with the production of IL 4 as measured by lymphokine bioassay and mRNA studies .
	manualset3
91536	7	399220	13	NULL	NULL	0	NULL	mRNA studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	IL 1 in combination with ionomycin ( iono/rIL 1 ) stimulated a proliferative response that was associated with the production of IL 4 as measured by lymphokine bioassay and mRNA studies .
	manualset3
91537	1	399221	13	NULL	NULL	0	NULL	IMPLICATIONS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	IMPLICATIONS : Complications , particularly when they involve organs other than just the heart , increase mortality and prolong the length of hospital stay after heart surgery , independent of a patient 's preoperative risk factors and the duration of cardiopulmonary bypass .
	manualset3
91538	2	399221	13	NULL	NULL	0	NULL	Complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	IMPLICATIONS : Complications , particularly when they involve organs other than just the heart , increase mortality and prolong the length of hospital stay after heart surgery , independent of a patient 's preoperative risk factors and the duration of cardiopulmonary bypass .
	manualset3
91539	3	399221	13	NULL	NULL	0	NULL	organs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	IMPLICATIONS : Complications , particularly when they involve organs other than just the heart , increase mortality and prolong the length of hospital stay after heart surgery , independent of a patient 's preoperative risk factors and the duration of cardiopulmonary bypass .
	manualset3
91540	4	399221	13	NULL	NULL	0	NULL	heart 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	IMPLICATIONS : Complications , particularly when they involve organs other than just the heart , increase mortality and prolong the length of hospital stay after heart surgery , independent of a patient 's preoperative risk factors and the duration of cardiopulmonary bypass .
	manualset3
91541	5	399221	13	NULL	NULL	0	NULL	 mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	IMPLICATIONS : Complications , particularly when they involve organs other than just the heart , increase mortality and prolong the length of hospital stay after heart surgery , independent of a patient 's preoperative risk factors and the duration of cardiopulmonary bypass .
	manualset3
91542	6	399221	13	NULL	NULL	0	NULL	length of hospital stay	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	IMPLICATIONS : Complications , particularly when they involve organs other than just the heart , increase mortality and prolong the length of hospital stay after heart surgery , independent of a patient 's preoperative risk factors and the duration of cardiopulmonary bypass .
	manualset3
91543	7	399221	13	NULL	NULL	0	NULL	 heart surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	IMPLICATIONS : Complications , particularly when they involve organs other than just the heart , increase mortality and prolong the length of hospital stay after heart surgery , independent of a patient 's preoperative risk factors and the duration of cardiopulmonary bypass .
	manualset3
91544	8	399221	13	NULL	NULL	0	NULL	patient 's preoperative risk factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	IMPLICATIONS : Complications , particularly when they involve organs other than just the heart , increase mortality and prolong the length of hospital stay after heart surgery , independent of a patient 's preoperative risk factors and the duration of cardiopulmonary bypass .
	manualset3
91545	9	399221	13	NULL	NULL	0	NULL	duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	IMPLICATIONS : Complications , particularly when they involve organs other than just the heart , increase mortality and prolong the length of hospital stay after heart surgery , independent of a patient 's preoperative risk factors and the duration of cardiopulmonary bypass .
	manualset3
91546	10	399221	13	NULL	NULL	0	NULL	cardiopulmonary bypass	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	IMPLICATIONS : Complications , particularly when they involve organs other than just the heart , increase mortality and prolong the length of hospital stay after heart surgery , independent of a patient 's preoperative risk factors and the duration of cardiopulmonary bypass .
	manualset3
91547	1	399222	13	NULL	NULL	0	NULL	IMPLICATIONS 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	IMPLICATIONS : We describe three patients with difficult airways in which fiberoptic endotracheal intubation was used to insert breathing tubes into the patients ' windpipes .
	manualset3
91548	2	399222	13	NULL	NULL	0	NULL	three 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	IMPLICATIONS : We describe three patients with difficult airways in which fiberoptic endotracheal intubation was used to insert breathing tubes into the patients ' windpipes .
	manualset3
91549	3	399222	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	IMPLICATIONS : We describe three patients with difficult airways in which fiberoptic endotracheal intubation was used to insert breathing tubes into the patients ' windpipes .
	manualset3
91550	4	399222	13	NULL	NULL	0	NULL	difficult airways	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	IMPLICATIONS : We describe three patients with difficult airways in which fiberoptic endotracheal intubation was used to insert breathing tubes into the patients ' windpipes .
	manualset3
91551	5	399222	13	NULL	NULL	0	NULL	 fiberoptic endotracheal intubation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	IMPLICATIONS : We describe three patients with difficult airways in which fiberoptic endotracheal intubation was used to insert breathing tubes into the patients ' windpipes .
	manualset3
91552	6	399222	13	NULL	NULL	0	NULL	breathing tubes	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	IMPLICATIONS : We describe three patients with difficult airways in which fiberoptic endotracheal intubation was used to insert breathing tubes into the patients ' windpipes .
	manualset3
91553	7	399222	13	NULL	NULL	0	NULL	 patients ' 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	IMPLICATIONS : We describe three patients with difficult airways in which fiberoptic endotracheal intubation was used to insert breathing tubes into the patients ' windpipes .
	manualset3
91554	8	399222	13	NULL	NULL	0	NULL	 windpipes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	IMPLICATIONS : We describe three patients with difficult airways in which fiberoptic endotracheal intubation was used to insert breathing tubes into the patients ' windpipes .
	manualset3
91555	1	399223	13	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	IN rats , a contractile threshold dose of ONO-802 was similar from day 15 to day 21 of pregnancy .
	manualset3
91556	2	399223	13	NULL	NULL	0	NULL	contractile threshold dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	IN rats , a contractile threshold dose of ONO-802 was similar from day 15 to day 21 of pregnancy .
	manualset3
91557	3	399223	13	NULL	NULL	0	NULL	 ONO-802	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	IN rats , a contractile threshold dose of ONO-802 was similar from day 15 to day 21 of pregnancy .
	manualset3
91558	4	399223	13	NULL	NULL	0	NULL	day 15 to day 21 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	IN rats , a contractile threshold dose of ONO-802 was similar from day 15 to day 21 of pregnancy .
	manualset3
91559	5	399223	13	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	IN rats , a contractile threshold dose of ONO-802 was similar from day 15 to day 21 of pregnancy .
	manualset3
91560	1	399224	13	NULL	NULL	0	NULL	INA	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	INA is usually localized in the uterine cervix , but , when multifocal lesions are present , the latter is almost always involved .
	manualset3
91561	2	399224	13	NULL	NULL	0	NULL	uterine cervix	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	INA is usually localized in the uterine cervix , but , when multifocal lesions are present , the latter is almost always involved .
	manualset3
91562	3	399224	13	NULL	NULL	0	NULL	 multifocal lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	INA is usually localized in the uterine cervix , but , when multifocal lesions are present , the latter is almost always involved .
	manualset3
91563	1	399225	13	NULL	NULL	0	NULL	INTRODUCTION	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	INTRODUCTION : Coronary artery disease ( CAD ) is one of the major causes of morbidity and mortality worldwide , exerting a huge economic burden .
	manualset3
91564	2	399225	13	NULL	NULL	0	NULL	Coronary artery disease ( CAD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	INTRODUCTION : Coronary artery disease ( CAD ) is one of the major causes of morbidity and mortality worldwide , exerting a huge economic burden .
	manualset3
91565	3	399225	13	NULL	NULL	NULL	NULL	one of the major causes of morbidity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	INTRODUCTION : Coronary artery disease ( CAD ) is one of the major causes of morbidity and mortality worldwide , exerting a huge economic burden .
	manualset3
91566	4	399225	13	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	INTRODUCTION : Coronary artery disease ( CAD ) is one of the major causes of morbidity and mortality worldwide , exerting a huge economic burden .
	manualset3
91567	5	399225	13	NULL	NULL	0	NULL	worldwide	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	INTRODUCTION : Coronary artery disease ( CAD ) is one of the major causes of morbidity and mortality worldwide , exerting a huge economic burden .
	manualset3
91568	6	399225	13	NULL	NULL	0	NULL	economic burden	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	INTRODUCTION : Coronary artery disease ( CAD ) is one of the major causes of morbidity and mortality worldwide , exerting a huge economic burden .
	manualset3
91569	1	399226	13	NULL	NULL	0	NULL	INTRODUCTION	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	INTRODUCTION : Juvenile polyposis syndrome ( JPS ) is a rare , autosomal dominant condition .
	manualset3
91570	2	399226	13	NULL	NULL	0	NULL	Juvenile polyposis syndrome ( JPS )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	INTRODUCTION : Juvenile polyposis syndrome ( JPS ) is a rare , autosomal dominant condition .
	manualset3
91571	3	399226	13	NULL	NULL	0	NULL	autosomal dominant condition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	INTRODUCTION : Juvenile polyposis syndrome ( JPS ) is a rare , autosomal dominant condition .
	manualset3
91572	1	399227	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( The study of iron metabolism in irradiated dogs with increased erythropoietic function ) .
	manualset3
91573	2	399227	13	NULL	NULL	0	NULL	 iron metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( The study of iron metabolism in irradiated dogs with increased erythropoietic function ) .
	manualset3
91574	3	399227	13	NULL	NULL	0	NULL	irradiated dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( The study of iron metabolism in irradiated dogs with increased erythropoietic function ) .
	manualset3
91575	4	399227	13	NULL	NULL	0	NULL	erythropoietic function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( The study of iron metabolism in irradiated dogs with increased erythropoietic function ) .
	manualset3
91576	1	399228	13	NULL	NULL	0	NULL	INTRODUCTION	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	INTRODUCTIONWe describe here a procedure for introducing loxP sites into the mammalian genome .
	manualset3
91577	2	399228	13	NULL	NULL	0	NULL	 procedure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	INTRODUCTIONWe describe here a procedure for introducing loxP sites into the mammalian genome .
	manualset3
91578	3	399228	13	NULL	NULL	0	NULL	loxP sites	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	INTRODUCTIONWe describe here a procedure for introducing loxP sites into the mammalian genome .
	manualset3
91579	4	399228	13	NULL	NULL	0	NULL	mammalian genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	INTRODUCTIONWe describe here a procedure for introducing loxP sites into the mammalian genome .
	manualset3
91580	1	399229	13	NULL	NULL	0	NULL	IOM	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	IOM is established as effective to predict an increased risk of the adverse outcomes of paraparesis , paraplegia , and quadriplegia in spinal surgery ( 4 Class I and 7 Class II studies ) .
	manualset3
91581	2	399229	13	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	IOM is established as effective to predict an increased risk of the adverse outcomes of paraparesis , paraplegia , and quadriplegia in spinal surgery ( 4 Class I and 7 Class II studies ) .
	manualset3
91582	3	399229	13	NULL	NULL	0	NULL	adverse outcomes of paraparesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	IOM is established as effective to predict an increased risk of the adverse outcomes of paraparesis , paraplegia , and quadriplegia in spinal surgery ( 4 Class I and 7 Class II studies ) .
	manualset3
91583	4	399229	13	NULL	NULL	0	NULL	paraplegia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	IOM is established as effective to predict an increased risk of the adverse outcomes of paraparesis , paraplegia , and quadriplegia in spinal surgery ( 4 Class I and 7 Class II studies ) .
	manualset3
91584	5	399229	13	NULL	NULL	0	NULL	quadriplegia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	IOM is established as effective to predict an increased risk of the adverse outcomes of paraparesis , paraplegia , and quadriplegia in spinal surgery ( 4 Class I and 7 Class II studies ) .
	manualset3
91585	6	399229	13	NULL	NULL	0	NULL	spinal surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	IOM is established as effective to predict an increased risk of the adverse outcomes of paraparesis , paraplegia , and quadriplegia in spinal surgery ( 4 Class I and 7 Class II studies ) .
	manualset3
91586	7	399229	13	NULL	NULL	0	NULL	4 Class I and 7 Class II studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	IOM is established as effective to predict an increased risk of the adverse outcomes of paraparesis , paraplegia , and quadriplegia in spinal surgery ( 4 Class I and 7 Class II studies ) .
	manualset3
91587	1	399230	13	NULL	NULL	0	NULL	IPANEMA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	IPANEMA , a research platform devoted to ancient and historical materials ( archaeology , cultural heritage , palaeontology and past environments ) , is currently being set up at the synchrotron facility SOLEIL ( Saint-Aubin , France ; SOLEIL opened to users in January 2008 ) .
	manualset3
91588	2	399230	13	NULL	NULL	0	NULL	a research platform	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	IPANEMA , a research platform devoted to ancient and historical materials ( archaeology , cultural heritage , palaeontology and past environments ) , is currently being set up at the synchrotron facility SOLEIL ( Saint-Aubin , France ; SOLEIL opened to users in January 2008 ) .
	manualset3
91589	3	399230	13	NULL	NULL	0	NULL	ancient materials	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	IPANEMA , a research platform devoted to ancient and historical materials ( archaeology , cultural heritage , palaeontology and past environments ) , is currently being set up at the synchrotron facility SOLEIL ( Saint-Aubin , France ; SOLEIL opened to users in January 2008 ) .
	manualset3
91590	4	399230	13	NULL	NULL	0	NULL	 historical materials	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	IPANEMA , a research platform devoted to ancient and historical materials ( archaeology , cultural heritage , palaeontology and past environments ) , is currently being set up at the synchrotron facility SOLEIL ( Saint-Aubin , France ; SOLEIL opened to users in January 2008 ) .
	manualset3
91591	5	399230	13	NULL	NULL	0	NULL	archaeology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	IPANEMA , a research platform devoted to ancient and historical materials ( archaeology , cultural heritage , palaeontology and past environments ) , is currently being set up at the synchrotron facility SOLEIL ( Saint-Aubin , France ; SOLEIL opened to users in January 2008 ) .
	manualset3
91592	6	399230	13	NULL	NULL	0	NULL	cultural heritage	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	IPANEMA , a research platform devoted to ancient and historical materials ( archaeology , cultural heritage , palaeontology and past environments ) , is currently being set up at the synchrotron facility SOLEIL ( Saint-Aubin , France ; SOLEIL opened to users in January 2008 ) .
	manualset3
91593	7	399230	13	NULL	NULL	0	NULL	palaeontology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	IPANEMA , a research platform devoted to ancient and historical materials ( archaeology , cultural heritage , palaeontology and past environments ) , is currently being set up at the synchrotron facility SOLEIL ( Saint-Aubin , France ; SOLEIL opened to users in January 2008 ) .
	manualset3
91594	8	399230	13	NULL	NULL	0	NULL	 past environments	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	IPANEMA , a research platform devoted to ancient and historical materials ( archaeology , cultural heritage , palaeontology and past environments ) , is currently being set up at the synchrotron facility SOLEIL ( Saint-Aubin , France ; SOLEIL opened to users in January 2008 ) .
	manualset3
91595	9	399230	13	NULL	NULL	0	NULL	synchrotron facility	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	IPANEMA , a research platform devoted to ancient and historical materials ( archaeology , cultural heritage , palaeontology and past environments ) , is currently being set up at the synchrotron facility SOLEIL ( Saint-Aubin , France ; SOLEIL opened to users in January 2008 ) .
	manualset3
91596	10	399230	13	NULL	NULL	0	NULL	SOLEIL 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	IPANEMA , a research platform devoted to ancient and historical materials ( archaeology , cultural heritage , palaeontology and past environments ) , is currently being set up at the synchrotron facility SOLEIL ( Saint-Aubin , France ; SOLEIL opened to users in January 2008 ) .
	manualset3
91597	11	399230	13	NULL	NULL	0	NULL	Saint-Aubin	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	IPANEMA , a research platform devoted to ancient and historical materials ( archaeology , cultural heritage , palaeontology and past environments ) , is currently being set up at the synchrotron facility SOLEIL ( Saint-Aubin , France ; SOLEIL opened to users in January 2008 ) .
	manualset3
91598	12	399230	13	NULL	NULL	0	NULL	France	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	IPANEMA , a research platform devoted to ancient and historical materials ( archaeology , cultural heritage , palaeontology and past environments ) , is currently being set up at the synchrotron facility SOLEIL ( Saint-Aubin , France ; SOLEIL opened to users in January 2008 ) .
	manualset3
91599	13	399230	13	NULL	NULL	0	NULL	SOLEIL 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	IPANEMA , a research platform devoted to ancient and historical materials ( archaeology , cultural heritage , palaeontology and past environments ) , is currently being set up at the synchrotron facility SOLEIL ( Saint-Aubin , France ; SOLEIL opened to users in January 2008 ) .
	manualset3
91600	14	399230	13	NULL	NULL	0	NULL	 users	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	IPANEMA , a research platform devoted to ancient and historical materials ( archaeology , cultural heritage , palaeontology and past environments ) , is currently being set up at the synchrotron facility SOLEIL ( Saint-Aubin , France ; SOLEIL opened to users in January 2008 ) .
	manualset3
91601	15	399230	13	NULL	NULL	0	NULL	January 2008 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	IPANEMA , a research platform devoted to ancient and historical materials ( archaeology , cultural heritage , palaeontology and past environments ) , is currently being set up at the synchrotron facility SOLEIL ( Saint-Aubin , France ; SOLEIL opened to users in January 2008 ) .
	manualset3
91602	1	399231	13	NULL	NULL	0	NULL	IRES-mediated translation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IRES-mediated translation of cellular messenger RNA operates in eIF2 - independent manner during stress .
	manualset3
91603	2	399231	13	NULL	NULL	0	NULL	cellular messenger RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	IRES-mediated translation of cellular messenger RNA operates in eIF2 - independent manner during stress .
	manualset3
91604	3	399231	13	NULL	NULL	0	NULL	eIF2 - independent manner	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IRES-mediated translation of cellular messenger RNA operates in eIF2 - independent manner during stress .
	manualset3
91605	4	399231	13	NULL	NULL	0	NULL	 stress 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	IRES-mediated translation of cellular messenger RNA operates in eIF2 - independent manner during stress .
	manualset3
91606	1	399232	13	NULL	NULL	NULL	NULL	Ibuprofen metabolite profiling 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ibuprofen metabolite profiling using a combination of SPE/column-trapping and HPLC-micro-coil NMR .
	manualset3
91607	2	399232	13	NULL	NULL	0	NULL	SPE/column-trapping	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ibuprofen metabolite profiling using a combination of SPE/column-trapping and HPLC-micro-coil NMR .
	manualset3
91608	3	399232	13	NULL	NULL	0	NULL	HPLC-micro-coil NMR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ibuprofen metabolite profiling using a combination of SPE/column-trapping and HPLC-micro-coil NMR .
	manualset3
91609	4	399232	13	NULL	NULL	0	NULL	 combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ibuprofen metabolite profiling using a combination of SPE/column-trapping and HPLC-micro-coil NMR .
	manualset3
91610	1	399233	13	NULL	NULL	0	NULL	Ibutilide-induced cardioversion 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ibutilide-induced cardioversion of atrial fibrillation during pregnancy .
	manualset3
91611	2	399233	13	NULL	NULL	0	NULL	atrial fibrillation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ibutilide-induced cardioversion of atrial fibrillation during pregnancy .
	manualset3
91612	3	399233	13	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ibutilide-induced cardioversion of atrial fibrillation during pregnancy .
	manualset3
91613	1	399234	13	NULL	NULL	0	NULL	 teaching	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( The teaching of anatomy in the United States ) .
	manualset3
91614	2	399234	13	NULL	NULL	0	NULL	anatomy	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( The teaching of anatomy in the United States ) .
	manualset3
91615	3	399234	13	NULL	NULL	0	NULL	United States	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( The teaching of anatomy in the United States ) .
	manualset3
91616	1	399235	13	NULL	NULL	0	NULL	Ictal blindness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ictal blindness was the solitary epileptic phenomenon in only two children .
	manualset3
91617	2	399235	13	NULL	NULL	0	NULL	solitary epileptic phenomenon	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ictal blindness was the solitary epileptic phenomenon in only two children .
	manualset3
91618	3	399235	13	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ictal blindness was the solitary epileptic phenomenon in only two children .
	manualset3
91619	4	399235	13	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ictal blindness was the solitary epileptic phenomenon in only two children .
	manualset3
91620	1	399236	13	NULL	NULL	0	NULL	reconstruction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ideally , reconstruction of lower extremity soft tissue defects includes not only an esthetically pleasing 3-dimensional shape and solid anchoring to the underlying structures to resist shear forces , but should also address the restoration of sensation .
	manualset3
91621	2	399236	13	NULL	NULL	0	NULL	lower extremity soft tissue defects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ideally , reconstruction of lower extremity soft tissue defects includes not only an esthetically pleasing 3-dimensional shape and solid anchoring to the underlying structures to resist shear forces , but should also address the restoration of sensation .
	manualset3
91622	3	399236	13	NULL	NULL	0	NULL	esthetically pleasing 3-dimensional shape	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Ideally , reconstruction of lower extremity soft tissue defects includes not only an esthetically pleasing 3-dimensional shape and solid anchoring to the underlying structures to resist shear forces , but should also address the restoration of sensation .
	manualset3
91623	4	399236	13	NULL	NULL	0	NULL	underlying structures	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Ideally , reconstruction of lower extremity soft tissue defects includes not only an esthetically pleasing 3-dimensional shape and solid anchoring to the underlying structures to resist shear forces , but should also address the restoration of sensation .
	manualset3
91624	5	399236	13	NULL	NULL	0	NULL	resist shear forces	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ideally , reconstruction of lower extremity soft tissue defects includes not only an esthetically pleasing 3-dimensional shape and solid anchoring to the underlying structures to resist shear forces , but should also address the restoration of sensation .
	manualset3
91625	6	399236	13	NULL	NULL	0	NULL	restoration of sensation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ideally , reconstruction of lower extremity soft tissue defects includes not only an esthetically pleasing 3-dimensional shape and solid anchoring to the underlying structures to resist shear forces , but should also address the restoration of sensation .
	manualset3
91626	1	399237	13	NULL	NULL	0	NULL	doctor 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Ideally , the doctor will inform the patient fully on the proposed treatment so as to assure the patient 's right to participate intelligently and freely in the decisions regarding his treatment .
	manualset3
91627	2	399237	13	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Ideally , the doctor will inform the patient fully on the proposed treatment so as to assure the patient 's right to participate intelligently and freely in the decisions regarding his treatment .
	manualset3
91628	3	399237	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ideally , the doctor will inform the patient fully on the proposed treatment so as to assure the patient 's right to participate intelligently and freely in the decisions regarding his treatment .
	manualset3
91629	4	399237	13	NULL	NULL	0	NULL	 patient 's	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Ideally , the doctor will inform the patient fully on the proposed treatment so as to assure the patient 's right to participate intelligently and freely in the decisions regarding his treatment .
	manualset3
91630	5	399237	13	NULL	NULL	NULL	NULL	decisions	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ideally , the doctor will inform the patient fully on the proposed treatment so as to assure the patient 's right to participate intelligently and freely in the decisions regarding his treatment .
	manualset3
91631	6	399237	13	NULL	NULL	0	NULL	 treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ideally , the doctor will inform the patient fully on the proposed treatment so as to assure the patient 's right to participate intelligently and freely in the decisions regarding his treatment .
	manualset3
91632	1	399238	13	NULL	NULL	0	NULL	diagnostic approach	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ideally the diagnostic approach to an individual patient will be highly tailored , not only in regard to the nature of the pulmonary lesion , but also to his or her overall medical and social situation .
	manualset3
91633	2	399238	13	NULL	NULL	0	NULL	individual patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Ideally the diagnostic approach to an individual patient will be highly tailored , not only in regard to the nature of the pulmonary lesion , but also to his or her overall medical and social situation .
	manualset3
91634	3	399238	13	NULL	NULL	0	NULL	nature of the pulmonary lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ideally the diagnostic approach to an individual patient will be highly tailored , not only in regard to the nature of the pulmonary lesion , but also to his or her overall medical and social situation .
	manualset3
91635	4	399238	13	NULL	NULL	0	NULL	medical situation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ideally the diagnostic approach to an individual patient will be highly tailored , not only in regard to the nature of the pulmonary lesion , but also to his or her overall medical and social situation .
	manualset3
91636	5	399238	13	NULL	NULL	NULL	NULL	social situation	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ideally the diagnostic approach to an individual patient will be highly tailored , not only in regard to the nature of the pulmonary lesion , but also to his or her overall medical and social situation .
	manualset3
91637	1	399239	13	NULL	NULL	0	NULL	Identical effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Identical effects of the peptides were observed in identified gastric-related and unlabeled DMV neurons .
	manualset3
91638	2	399239	13	NULL	NULL	0	NULL	peptides 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Identical effects of the peptides were observed in identified gastric-related and unlabeled DMV neurons .
	manualset3
91639	3	399239	13	NULL	NULL	0	NULL	gastric-related neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Identical effects of the peptides were observed in identified gastric-related and unlabeled DMV neurons .
	manualset3
91640	4	399239	13	NULL	NULL	0	NULL	unlabeled DMV neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Identical effects of the peptides were observed in identified gastric-related and unlabeled DMV neurons .
	manualset3
91641	1	399240	13	NULL	NULL	0	NULL	Identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification and characterization of a rat hepatic oncofetal membrane glycoprotein .
	manualset3
91642	2	399240	13	NULL	NULL	0	NULL	characterization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification and characterization of a rat hepatic oncofetal membrane glycoprotein .
	manualset3
91643	3	399240	13	NULL	NULL	0	NULL	rat hepatic oncofetal membrane glycoprotein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification and characterization of a rat hepatic oncofetal membrane glycoprotein .
	manualset3
91644	1	399241	13	NULL	NULL	0	NULL	Identification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification and characterization of metal ion binding sites in RNA .
	manualset3
91645	2	399241	13	NULL	NULL	0	NULL	characterization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification and characterization of metal ion binding sites in RNA .
	manualset3
91646	3	399241	13	NULL	NULL	0	NULL	 metal ion binding sites in RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification and characterization of metal ion binding sites in RNA .
	manualset3
91647	1	399242	13	NULL	NULL	0	NULL	Identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification and molecular mapping of two QTLs with major effects for resistance to Fusarium head blight in wheat .
	manualset3
91648	2	399242	13	NULL	NULL	0	NULL	molecular mapping	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification and molecular mapping of two QTLs with major effects for resistance to Fusarium head blight in wheat .
	manualset3
91649	3	399242	13	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification and molecular mapping of two QTLs with major effects for resistance to Fusarium head blight in wheat .
	manualset3
91650	4	399242	13	NULL	NULL	0	NULL	QTLs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification and molecular mapping of two QTLs with major effects for resistance to Fusarium head blight in wheat .
	manualset3
91651	5	399242	13	NULL	NULL	0	NULL	major effects for resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification and molecular mapping of two QTLs with major effects for resistance to Fusarium head blight in wheat .
	manualset3
91652	6	399242	13	NULL	NULL	0	NULL	Fusarium head blight	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification and molecular mapping of two QTLs with major effects for resistance to Fusarium head blight in wheat .
	manualset3
91653	7	399242	13	NULL	NULL	0	NULL	wheat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification and molecular mapping of two QTLs with major effects for resistance to Fusarium head blight in wheat .
	manualset3
91654	1	399243	13	NULL	NULL	0	NULL	teaching role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The teaching role of the midwife ) .
	manualset3
91655	2	399243	13	NULL	NULL	0	NULL	midwife	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( The teaching role of the midwife ) .
	manualset3
91656	1	399244	13	NULL	NULL	0	NULL	Identification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification and nucleotide sequence of the heat shock protein 60 ( GroEL ) gene of Bacteroides forsythus .
	manualset3
91657	2	399244	13	NULL	NULL	NULL	NULL	nucleotide sequence of the heat shock protein 60 ( GroEL ) gene 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Identification and nucleotide sequence of the heat shock protein 60 ( GroEL ) gene of Bacteroides forsythus .
	manualset3
91658	3	399244	13	NULL	NULL	0	NULL	Bacteroides forsythus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification and nucleotide sequence of the heat shock protein 60 ( GroEL ) gene of Bacteroides forsythus .
	manualset3
91659	1	399245	13	NULL	NULL	0	NULL	Identification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of Acinetobacter species isolated from clinical specimens by amplified ribosomal DNA restriction analysis .
	manualset3
91660	2	399245	13	NULL	NULL	0	NULL	Acinetobacter species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of Acinetobacter species isolated from clinical specimens by amplified ribosomal DNA restriction analysis .
	manualset3
91661	3	399245	13	NULL	NULL	NULL	NULL	clinical specimens 	AnatomicalPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Identification of Acinetobacter species isolated from clinical specimens by amplified ribosomal DNA restriction analysis .
	manualset3
91662	4	399245	13	NULL	NULL	0	NULL	amplified ribosomal DNA restriction analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of Acinetobacter species isolated from clinical specimens by amplified ribosomal DNA restriction analysis .
	manualset3
91663	1	399246	13	NULL	NULL	0	NULL	Identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of Candida dubliniensis based on temperature and utilization of xylose and alpha-methyl-D-glucoside as determined with the API 20C AUX and vitek YBC systems .
	manualset3
91664	2	399246	13	NULL	NULL	0	NULL	Candida dubliniensis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of Candida dubliniensis based on temperature and utilization of xylose and alpha-methyl-D-glucoside as determined with the API 20C AUX and vitek YBC systems .
	manualset3
91665	3	399246	13	NULL	NULL	0	NULL	temperature	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of Candida dubliniensis based on temperature and utilization of xylose and alpha-methyl-D-glucoside as determined with the API 20C AUX and vitek YBC systems .
	manualset3
91666	4	399246	13	NULL	NULL	0	NULL	utilization of xylose	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of Candida dubliniensis based on temperature and utilization of xylose and alpha-methyl-D-glucoside as determined with the API 20C AUX and vitek YBC systems .
	manualset3
91667	5	399246	13	NULL	NULL	0	NULL	 utilization of alpha-methyl-D-glucoside	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of Candida dubliniensis based on temperature and utilization of xylose and alpha-methyl-D-glucoside as determined with the API 20C AUX and vitek YBC systems .
	manualset3
91668	6	399246	13	NULL	NULL	0	NULL	API 20C AUX	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of Candida dubliniensis based on temperature and utilization of xylose and alpha-methyl-D-glucoside as determined with the API 20C AUX and vitek YBC systems .
	manualset3
91669	7	399246	13	NULL	NULL	0	NULL	vitek YBC systems	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of Candida dubliniensis based on temperature and utilization of xylose and alpha-methyl-D-glucoside as determined with the API 20C AUX and vitek YBC systems .
	manualset3
91670	1	399247	13	NULL	NULL	0	NULL	Identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of NEEP21 as a - amyloid precursor protein-interacting protein in vivo that modulates amyloidogenic processing in vitro .
	manualset3
91671	2	399247	13	NULL	NULL	0	NULL	NEEP21	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of NEEP21 as a - amyloid precursor protein-interacting protein in vivo that modulates amyloidogenic processing in vitro .
	manualset3
91672	3	399247	13	NULL	NULL	0	NULL	a - amyloid precursor protein-interacting protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of NEEP21 as a - amyloid precursor protein-interacting protein in vivo that modulates amyloidogenic processing in vitro .
	manualset3
98571	4	399247	13	NULL	NULL	NULL	NULL	amyloidogenic processing	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Identification of NEEP21 as a - amyloid precursor protein-interacting protein in vivo that modulates amyloidogenic processing in vitro .
	manualset3
91673	1	399248	13	NULL	NULL	0	NULL	Identification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of Plum pox virus Determinants Implicated in Specific Interactions with Different Prunus spp .
	manualset3
91674	2	399248	13	NULL	NULL	0	NULL	Plum pox virus Determinants	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of Plum pox virus Determinants Implicated in Specific Interactions with Different Prunus spp .
	manualset3
91675	3	399248	13	NULL	NULL	0	NULL	Specific Interactions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of Plum pox virus Determinants Implicated in Specific Interactions with Different Prunus spp .
	manualset3
91676	4	399248	13	NULL	NULL	0	NULL	Different Prunus spp	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of Plum pox virus Determinants Implicated in Specific Interactions with Different Prunus spp .
	manualset3
91677	1	399249	13	NULL	NULL	0	NULL	Identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of SOX3 as an XX male sex reversal gene in mice and humans .
	manualset3
91678	2	399249	13	NULL	NULL	0	NULL	SOX3	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of SOX3 as an XX male sex reversal gene in mice and humans .
	manualset3
91679	3	399249	13	NULL	NULL	0	NULL	XX male sex reversal gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of SOX3 as an XX male sex reversal gene in mice and humans .
	manualset3
91680	4	399249	13	NULL	NULL	0	NULL	 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of SOX3 as an XX male sex reversal gene in mice and humans .
	manualset3
91681	5	399249	13	NULL	NULL	0	NULL	humans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of SOX3 as an XX male sex reversal gene in mice and humans .
	manualset3
91682	1	399250	13	NULL	NULL	0	NULL	Identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of Staphylococcus aureus ( food laboratories ) : microscopic observation , catalase activity , coagulase production , thermonuclease production , and ( optional ) lysostaphin sensitivity .
	manualset3
91683	2	399250	13	NULL	NULL	0	NULL	Staphylococcus aureus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of Staphylococcus aureus ( food laboratories ) : microscopic observation , catalase activity , coagulase production , thermonuclease production , and ( optional ) lysostaphin sensitivity .
	manualset3
91684	3	399250	13	NULL	NULL	0	NULL	food laboratories	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of Staphylococcus aureus ( food laboratories ) : microscopic observation , catalase activity , coagulase production , thermonuclease production , and ( optional ) lysostaphin sensitivity .
	manualset3
91685	4	399250	13	NULL	NULL	0	NULL	microscopic observation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of Staphylococcus aureus ( food laboratories ) : microscopic observation , catalase activity , coagulase production , thermonuclease production , and ( optional ) lysostaphin sensitivity .
	manualset3
91686	5	399250	13	NULL	NULL	0	NULL	catalase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of Staphylococcus aureus ( food laboratories ) : microscopic observation , catalase activity , coagulase production , thermonuclease production , and ( optional ) lysostaphin sensitivity .
	manualset3
91687	6	399250	13	NULL	NULL	0	NULL	 coagulase production 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of Staphylococcus aureus ( food laboratories ) : microscopic observation , catalase activity , coagulase production , thermonuclease production , and ( optional ) lysostaphin sensitivity .
	manualset3
91688	7	399250	13	NULL	NULL	0	NULL	thermonuclease production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of Staphylococcus aureus ( food laboratories ) : microscopic observation , catalase activity , coagulase production , thermonuclease production , and ( optional ) lysostaphin sensitivity .
	manualset3
91689	8	399250	13	NULL	NULL	0	NULL	lysostaphin sensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of Staphylococcus aureus ( food laboratories ) : microscopic observation , catalase activity , coagulase production , thermonuclease production , and ( optional ) lysostaphin sensitivity .
	manualset3
91690	1	399251	13	NULL	NULL	0	NULL	Identification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of a diacylglycerol acyltransferase 2 gene involved in pheromone biosynthesis activating neuropeptide stimulated pheromone production in Bombyx mori .
	manualset3
91691	2	399251	13	NULL	NULL	0	NULL	diacylglycerol acyltransferase 2 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of a diacylglycerol acyltransferase 2 gene involved in pheromone biosynthesis activating neuropeptide stimulated pheromone production in Bombyx mori .
	manualset3
91692	3	399251	13	NULL	NULL	0	NULL	pheromone biosynthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of a diacylglycerol acyltransferase 2 gene involved in pheromone biosynthesis activating neuropeptide stimulated pheromone production in Bombyx mori .
	manualset3
91693	4	399251	13	NULL	NULL	0	NULL	neuropeptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of a diacylglycerol acyltransferase 2 gene involved in pheromone biosynthesis activating neuropeptide stimulated pheromone production in Bombyx mori .
	manualset3
91694	5	399251	13	NULL	NULL	0	NULL	pheromone production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of a diacylglycerol acyltransferase 2 gene involved in pheromone biosynthesis activating neuropeptide stimulated pheromone production in Bombyx mori .
	manualset3
91695	6	399251	13	NULL	NULL	0	NULL	Bombyx mori 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of a diacylglycerol acyltransferase 2 gene involved in pheromone biosynthesis activating neuropeptide stimulated pheromone production in Bombyx mori .
	manualset3
91696	1	399252	13	NULL	NULL	0	NULL	Identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of a dominant form in a blood smear provides a clue to diagnosis .
	manualset3
91697	2	399252	13	NULL	NULL	0	NULL	dominant form	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of a dominant form in a blood smear provides a clue to diagnosis .
	manualset3
91698	3	399252	13	NULL	NULL	0	NULL	blood smear	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of a dominant form in a blood smear provides a clue to diagnosis .
	manualset3
91699	4	399252	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of a dominant form in a blood smear provides a clue to diagnosis .
	manualset3
91700	5	399252	13	NULL	NULL	0	NULL	clue	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of a dominant form in a blood smear provides a clue to diagnosis .
	manualset3
91701	1	399253	13	NULL	NULL	0	NULL	technique of obtaining gastric juice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( The technique of obtaining gastric juice from dogs with a small Pavlov 's pouch ) .
	manualset3
91702	2	399253	13	NULL	NULL	0	NULL	dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( The technique of obtaining gastric juice from dogs with a small Pavlov 's pouch ) .
	manualset3
91703	3	399253	13	NULL	NULL	0	NULL	small Pavlov 's pouch	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( The technique of obtaining gastric juice from dogs with a small Pavlov 's pouch ) .
	manualset3
91704	1	399254	13	NULL	NULL	0	NULL	Identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of a novel proinflammatory human skin-homing V9V2 T cell subset with a potential role in psoriasis .
	manualset3
91705	2	399254	13	NULL	NULL	0	NULL	a novel proinflammatory human skin-homing V9V2 T cell subset	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of a novel proinflammatory human skin-homing V9V2 T cell subset with a potential role in psoriasis .
	manualset3
91706	3	399254	13	NULL	NULL	0	NULL	potential role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of a novel proinflammatory human skin-homing V9V2 T cell subset with a potential role in psoriasis .
	manualset3
91707	4	399254	13	NULL	NULL	0	NULL	psoriasis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of a novel proinflammatory human skin-homing V9V2 T cell subset with a potential role in psoriasis .
	manualset3
91708	1	399255	13	NULL	NULL	0	NULL	Identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of a protein that interacts with the golli-myelin basic protein and with nuclear LIM interactor in the nervous system .
	manualset3
91709	2	399255	13	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of a protein that interacts with the golli-myelin basic protein and with nuclear LIM interactor in the nervous system .
	manualset3
91710	3	399255	13	NULL	NULL	0	NULL	 golli-myelin basic protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of a protein that interacts with the golli-myelin basic protein and with nuclear LIM interactor in the nervous system .
	manualset3
91711	4	399255	13	NULL	NULL	0	NULL	nuclear LIM interactor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of a protein that interacts with the golli-myelin basic protein and with nuclear LIM interactor in the nervous system .
	manualset3
91712	5	399255	13	NULL	NULL	0	NULL	nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of a protein that interacts with the golli-myelin basic protein and with nuclear LIM interactor in the nervous system .
	manualset3
91713	1	399256	13	NULL	NULL	0	NULL	Identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of additional target sites downstream of COX may benefit the ) 27 , 000 patients whom die annually from cirrhosis in the United States alone .
	manualset3
91714	2	399256	13	NULL	NULL	0	NULL	 target sites downstream of COX	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of additional target sites downstream of COX may benefit the ) 27 , 000 patients whom die annually from cirrhosis in the United States alone .
	manualset3
91715	3	399256	13	NULL	NULL	0	NULL	 benefit	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of additional target sites downstream of COX may benefit the ) 27 , 000 patients whom die annually from cirrhosis in the United States alone .
	manualset3
91716	4	399256	13	NULL	NULL	0	NULL	27 , 000	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of additional target sites downstream of COX may benefit the ) 27 , 000 patients whom die annually from cirrhosis in the United States alone .
	manualset3
91717	5	399256	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of additional target sites downstream of COX may benefit the ) 27 , 000 patients whom die annually from cirrhosis in the United States alone .
	manualset3
91719	7	399256	13	NULL	NULL	0	NULL	cirrhosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of additional target sites downstream of COX may benefit the ) 27 , 000 patients whom die annually from cirrhosis in the United States alone .
	manualset3
91720	8	399256	13	NULL	NULL	0	NULL	United States	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of additional target sites downstream of COX may benefit the ) 27 , 000 patients whom die annually from cirrhosis in the United States alone .
	manualset3
91721	1	399257	13	NULL	NULL	0	NULL	Identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of amino acid residues essential for the substrate specificity of Flavobacterium sp .
	manualset3
91722	2	399257	13	NULL	NULL	0	NULL	 amino acid residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of amino acid residues essential for the substrate specificity of Flavobacterium sp .
	manualset3
91723	3	399257	13	NULL	NULL	0	NULL	substrate specificity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of amino acid residues essential for the substrate specificity of Flavobacterium sp .
	manualset3
91724	4	399257	13	NULL	NULL	0	NULL	Flavobacterium sp	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of amino acid residues essential for the substrate specificity of Flavobacterium sp .
	manualset3
91725	1	399258	13	NULL	NULL	0	NULL	Identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of beta-hemolytic streptococci isolated from hospitalized children in Baghdad .
	manualset3
91726	2	399258	13	NULL	NULL	0	NULL	beta-hemolytic streptococci 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of beta-hemolytic streptococci isolated from hospitalized children in Baghdad .
	manualset3
91727	3	399258	13	NULL	NULL	NULL	NULL	children	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Identification of beta-hemolytic streptococci isolated from hospitalized children in Baghdad .
	manualset3
91728	4	399258	13	NULL	NULL	0	NULL	Baghdad	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of beta-hemolytic streptococci isolated from hospitalized children in Baghdad .
	manualset3
91729	1	399259	13	NULL	NULL	0	NULL	Identification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of beta adrenoreceptors during thymocyte ontogeny in mice .
	manualset3
91730	2	399259	13	NULL	NULL	0	NULL	beta adrenoreceptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of beta adrenoreceptors during thymocyte ontogeny in mice .
	manualset3
91731	3	399259	13	NULL	NULL	0	NULL	thymocyte ontogeny	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of beta adrenoreceptors during thymocyte ontogeny in mice .
	manualset3
91732	4	399259	13	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of beta adrenoreceptors during thymocyte ontogeny in mice .
	manualset3
91733	1	399260	13	NULL	NULL	0	NULL	Identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of bovine brain calcium binding proteins .
	manualset3
91734	2	399260	13	NULL	NULL	0	NULL	bovine brain calcium binding proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of bovine brain calcium binding proteins .
	manualset3
91735	1	399261	13	NULL	NULL	0	NULL	Identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of genetic parameters associated with disease progression in plasma cell myeloma .
	manualset3
91736	2	399261	13	NULL	NULL	0	NULL	genetic parameters	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of genetic parameters associated with disease progression in plasma cell myeloma .
	manualset3
91737	3	399261	13	NULL	NULL	0	NULL	disease progression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of genetic parameters associated with disease progression in plasma cell myeloma .
	manualset3
91738	4	399261	13	NULL	NULL	0	NULL	plasma cell myeloma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of genetic parameters associated with disease progression in plasma cell myeloma .
	manualset3
91739	1	399262	13	NULL	NULL	0	NULL	Identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of homocystinuric newborns is hindered by the pitfalls of neonatal screening programs .
	manualset3
91740	2	399262	13	NULL	NULL	0	NULL	homocystinuric newborns	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of homocystinuric newborns is hindered by the pitfalls of neonatal screening programs .
	manualset3
91741	3	399262	13	NULL	NULL	0	NULL	 neonatal screening programs	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of homocystinuric newborns is hindered by the pitfalls of neonatal screening programs .
	manualset3
91743	1	399263	13	NULL	NULL	0	NULL	aprophen	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( The use of aprophen in internal diseases ) .
	manualset3
91744	2	399263	13	NULL	NULL	0	NULL	 internal diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( The use of aprophen in internal diseases ) .
	manualset3
91745	1	399264	13	NULL	NULL	0	NULL	Identification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of intimin alleles in pathogenic Escherichia coli by PCR-restriction fragment length polymorphism analysis .
	manualset3
91746	2	399264	13	NULL	NULL	0	NULL	 intimin alleles 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of intimin alleles in pathogenic Escherichia coli by PCR-restriction fragment length polymorphism analysis .
	manualset3
91747	3	399264	13	NULL	NULL	0	NULL	pathogenic Escherichia coli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of intimin alleles in pathogenic Escherichia coli by PCR-restriction fragment length polymorphism analysis .
	manualset3
91749	4	399264	13	NULL	NULL	0	NULL	PCR-restriction fragment length polymorphism analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of intimin alleles in pathogenic Escherichia coli by PCR-restriction fragment length polymorphism analysis .
	manualset3
91750	1	399265	13	NULL	NULL	0	NULL	Identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of macrophages in sections of rabbit lung using acetoacetylated lipoproteins .
	manualset3
91751	2	399265	13	NULL	NULL	0	NULL	macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of macrophages in sections of rabbit lung using acetoacetylated lipoproteins .
	manualset3
91752	3	399265	13	NULL	NULL	0	NULL	sections of rabbit lung 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of macrophages in sections of rabbit lung using acetoacetylated lipoproteins .
	manualset3
91753	4	399265	13	NULL	NULL	0	NULL	acetoacetylated lipoproteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of macrophages in sections of rabbit lung using acetoacetylated lipoproteins .
	manualset3
91754	1	399266	13	NULL	NULL	0	NULL	Identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of muscle-specific calpain and beta-sarcoglycan genes in progressive autosomal recessive muscular dystrophies .
	manualset3
91755	2	399266	13	NULL	NULL	NULL	NULL	muscle-specific calpain gene	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Identification of muscle-specific calpain and beta-sarcoglycan genes in progressive autosomal recessive muscular dystrophies .
	manualset3
91756	3	399266	13	NULL	NULL	NULL	NULL	beta-sarcoglycan gene	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Identification of muscle-specific calpain and beta-sarcoglycan genes in progressive autosomal recessive muscular dystrophies .
	manualset3
91757	4	399266	13	NULL	NULL	0	NULL	 progressive autosomal recessive muscular dystrophies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of muscle-specific calpain and beta-sarcoglycan genes in progressive autosomal recessive muscular dystrophies .
	manualset3
91758	1	399267	13	NULL	NULL	0	NULL	Identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of several clinical isolates of dermatophytes based on the nucleotide sequence of internal transcribed spacer 1 ( ITS 1 ) in nuclear ribosomal DNA .
	manualset3
91759	2	399267	13	NULL	NULL	0	NULL	clinical isolates of dermatophytes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of several clinical isolates of dermatophytes based on the nucleotide sequence of internal transcribed spacer 1 ( ITS 1 ) in nuclear ribosomal DNA .
	manualset3
91760	3	399267	13	NULL	NULL	0	NULL	nucleotide sequence of internal transcribed spacer 1 ( ITS 1 ) 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of several clinical isolates of dermatophytes based on the nucleotide sequence of internal transcribed spacer 1 ( ITS 1 ) in nuclear ribosomal DNA .
	manualset3
91761	4	399267	13	NULL	NULL	0	NULL	nuclear ribosomal DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of several clinical isolates of dermatophytes based on the nucleotide sequence of internal transcribed spacer 1 ( ITS 1 ) in nuclear ribosomal DNA .
	manualset3
91762	1	399268	13	NULL	NULL	0	NULL	Identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of the gene encoding sulfopyruvate decarboxylase , an enzyme involved in biosynthesis of coenzyme M .
	manualset3
91763	2	399268	13	NULL	NULL	NULL	NULL	gene 	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Identification of the gene encoding sulfopyruvate decarboxylase , an enzyme involved in biosynthesis of coenzyme M .
	manualset3
91764	4	399268	13	NULL	NULL	NULL	NULL	enzyme	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Identification of the gene encoding sulfopyruvate decarboxylase , an enzyme involved in biosynthesis of coenzyme M .
	manualset3
92466	5	399268	13	NULL	NULL	NULL	NULL	 biosynthesis of coenzyme M	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Identification of the gene encoding sulfopyruvate decarboxylase , an enzyme involved in biosynthesis of coenzyme M .
	manualset3
92471	3	399268	13	NULL	NULL	0	NULL	sulfopyruvate decarboxylase	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of the gene encoding sulfopyruvate decarboxylase , an enzyme involved in biosynthesis of coenzyme M .
	manualset3
91765	1	399269	13	NULL	NULL	0	NULL	Identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of the molecular lesions covering the gamut of MFS clinical variability should allow the construction of genotype/phenotype correlations .
	manualset3
91766	2	399269	13	NULL	NULL	0	NULL	molecular lesions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of the molecular lesions covering the gamut of MFS clinical variability should allow the construction of genotype/phenotype correlations .
	manualset3
91767	3	399269	13	NULL	NULL	0	NULL	gamut of MFS clinical variability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of the molecular lesions covering the gamut of MFS clinical variability should allow the construction of genotype/phenotype correlations .
	manualset3
91768	4	399269	13	NULL	NULL	0	NULL	construction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of the molecular lesions covering the gamut of MFS clinical variability should allow the construction of genotype/phenotype correlations .
	manualset3
91769	5	399269	13	NULL	NULL	0	NULL	genotype/phenotype correlations 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of the molecular lesions covering the gamut of MFS clinical variability should allow the construction of genotype/phenotype correlations .
	manualset3
91770	1	399270	13	NULL	NULL	0	NULL	Identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of the molecular mechanisms of VSMC activation is crucial in understanding the initiation of vascular restenosis .
	manualset3
91771	2	399270	13	NULL	NULL	0	NULL	molecular mechanisms 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of the molecular mechanisms of VSMC activation is crucial in understanding the initiation of vascular restenosis .
	manualset3
91772	3	399270	13	NULL	NULL	0	NULL	VSMC activation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of the molecular mechanisms of VSMC activation is crucial in understanding the initiation of vascular restenosis .
	manualset3
91773	4	399270	13	NULL	NULL	0	NULL	initiation of vascular restenosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of the molecular mechanisms of VSMC activation is crucial in understanding the initiation of vascular restenosis .
	manualset3
91774	1	399271	13	NULL	NULL	0	NULL	Identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of these proteins and their binding affinities for Abeta are needed to assess their potential role in the pathogenesis of Alzheimer 's disease .
	manualset3
91775	2	399271	13	NULL	NULL	0	NULL	 proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of these proteins and their binding affinities for Abeta are needed to assess their potential role in the pathogenesis of Alzheimer 's disease .
	manualset3
91776	3	399271	13	NULL	NULL	0	NULL	binding affinities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of these proteins and their binding affinities for Abeta are needed to assess their potential role in the pathogenesis of Alzheimer 's disease .
	manualset3
91777	4	399271	13	NULL	NULL	0	NULL	 Abeta 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of these proteins and their binding affinities for Abeta are needed to assess their potential role in the pathogenesis of Alzheimer 's disease .
	manualset3
91778	5	399271	13	NULL	NULL	0	NULL	potential role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of these proteins and their binding affinities for Abeta are needed to assess their potential role in the pathogenesis of Alzheimer 's disease .
	manualset3
91779	6	399271	13	NULL	NULL	0	NULL	 pathogenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of these proteins and their binding affinities for Abeta are needed to assess their potential role in the pathogenesis of Alzheimer 's disease .
	manualset3
91780	7	399271	13	NULL	NULL	0	NULL	Alzheimer 's disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of these proteins and their binding affinities for Abeta are needed to assess their potential role in the pathogenesis of Alzheimer 's disease .
	manualset3
91781	1	399272	13	NULL	NULL	0	NULL	Anemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Anemia in chronic renal insufficiency and chronic failure ) .
	manualset3
91782	2	399272	13	NULL	NULL	0	NULL	chronic renal insufficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Anemia in chronic renal insufficiency and chronic failure ) .
	manualset3
91783	3	399272	13	NULL	NULL	0	NULL	chronic failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Anemia in chronic renal insufficiency and chronic failure ) .
	manualset3
91784	1	399273	13	NULL	NULL	0	NULL	corticosteroids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( The use of corticosteroids in intensive care unit ( author 's transl ) ) .
	manualset3
91785	2	399273	13	NULL	NULL	0	NULL	intensive care unit	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( The use of corticosteroids in intensive care unit ( author 's transl ) ) .
	manualset3
91786	3	399273	13	NULL	NULL	0	NULL	author 's	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( The use of corticosteroids in intensive care unit ( author 's transl ) ) .
	manualset3
91787	1	399274	13	NULL	NULL	0	NULL	Identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of two regulatory elements within the promoter region of the mouse connexin 43 gene .
	manualset3
91788	2	399274	13	NULL	NULL	0	NULL	two regulatory elements	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of two regulatory elements within the promoter region of the mouse connexin 43 gene .
	manualset3
91789	3	399274	13	NULL	NULL	0	NULL	promoter region of the mouse connexin 43 gene	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of two regulatory elements within the promoter region of the mouse connexin 43 gene .
	manualset3
91790	1	399275	13	NULL	NULL	0	NULL	Identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of very few cynomolgus monkey-specific framework region residues suggests a role for cynomolgus monkey antibodies as donators of variable regions to chimeric monoclonal antibodies for utilisation in human therapy with human constant ( C ) regions .
	manualset3
91791	2	399275	13	NULL	NULL	0	NULL	 cynomolgus monkey-specific framework region residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of very few cynomolgus monkey-specific framework region residues suggests a role for cynomolgus monkey antibodies as donators of variable regions to chimeric monoclonal antibodies for utilisation in human therapy with human constant ( C ) regions .
	manualset3
91792	3	399275	13	NULL	NULL	0	NULL	role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of very few cynomolgus monkey-specific framework region residues suggests a role for cynomolgus monkey antibodies as donators of variable regions to chimeric monoclonal antibodies for utilisation in human therapy with human constant ( C ) regions .
	manualset3
91793	4	399275	13	NULL	NULL	NULL	NULL	cynomolgus monkey antibodies	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Identification of very few cynomolgus monkey-specific framework region residues suggests a role for cynomolgus monkey antibodies as donators of variable regions to chimeric monoclonal antibodies for utilisation in human therapy with human constant ( C ) regions .
	manualset3
91794	5	399275	13	NULL	NULL	0	NULL	donators of variable regions	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of very few cynomolgus monkey-specific framework region residues suggests a role for cynomolgus monkey antibodies as donators of variable regions to chimeric monoclonal antibodies for utilisation in human therapy with human constant ( C ) regions .
	manualset3
91795	6	399275	13	NULL	NULL	0	NULL	chimeric monoclonal antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of very few cynomolgus monkey-specific framework region residues suggests a role for cynomolgus monkey antibodies as donators of variable regions to chimeric monoclonal antibodies for utilisation in human therapy with human constant ( C ) regions .
	manualset3
91796	7	399275	13	NULL	NULL	0	NULL	utilisation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of very few cynomolgus monkey-specific framework region residues suggests a role for cynomolgus monkey antibodies as donators of variable regions to chimeric monoclonal antibodies for utilisation in human therapy with human constant ( C ) regions .
	manualset3
91797	8	399275	13	NULL	NULL	0	NULL	human therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of very few cynomolgus monkey-specific framework region residues suggests a role for cynomolgus monkey antibodies as donators of variable regions to chimeric monoclonal antibodies for utilisation in human therapy with human constant ( C ) regions .
	manualset3
91798	9	399275	13	NULL	NULL	NULL	NULL	human constant ( C ) regions	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Identification of very few cynomolgus monkey-specific framework region residues suggests a role for cynomolgus monkey antibodies as donators of variable regions to chimeric monoclonal antibodies for utilisation in human therapy with human constant ( C ) regions .
	manualset3
91799	1	399276	13	NULL	NULL	0	NULL	Identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of viruses in a study of acute respiratory tract infection in children from Uruguay .
	manualset3
91800	2	399276	13	NULL	NULL	0	NULL	viruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of viruses in a study of acute respiratory tract infection in children from Uruguay .
	manualset3
91801	3	399276	13	NULL	NULL	NULL	NULL	study 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Identification of viruses in a study of acute respiratory tract infection in children from Uruguay .
	manualset3
91802	4	399276	13	NULL	NULL	0	NULL	acute respiratory tract infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of viruses in a study of acute respiratory tract infection in children from Uruguay .
	manualset3
91803	5	399276	13	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of viruses in a study of acute respiratory tract infection in children from Uruguay .
	manualset3
91804	6	399276	13	NULL	NULL	0	NULL	Uruguay	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of viruses in a study of acute respiratory tract infection in children from Uruguay .
	manualset3
91805	1	399277	13	NULL	NULL	0	NULL	epitopes	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Identifying epitopes that elicit a major histocompatibility complex ( MHC ) - restricted T-cell response is critical for designing vaccines for infectious diseases and cancers .
	manualset3
91806	2	399277	13	NULL	NULL	0	NULL	major histocompatibility complex ( MHC ) - restricted T-cell response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Identifying epitopes that elicit a major histocompatibility complex ( MHC ) - restricted T-cell response is critical for designing vaccines for infectious diseases and cancers .
	manualset3
91807	3	399277	13	NULL	NULL	0	NULL	designing vaccines	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Identifying epitopes that elicit a major histocompatibility complex ( MHC ) - restricted T-cell response is critical for designing vaccines for infectious diseases and cancers .
	manualset3
91808	4	399277	13	NULL	NULL	0	NULL	infectious diseases 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Identifying epitopes that elicit a major histocompatibility complex ( MHC ) - restricted T-cell response is critical for designing vaccines for infectious diseases and cancers .
	manualset3
91809	5	399277	13	NULL	NULL	0	NULL	cancers	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Identifying epitopes that elicit a major histocompatibility complex ( MHC ) - restricted T-cell response is critical for designing vaccines for infectious diseases and cancers .
	manualset3
91810	1	399278	13	NULL	NULL	0	NULL	hypoxemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Identifying hypoxemia in children admitted for adenotonsillectomy .
	manualset3
91811	2	399278	13	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Identifying hypoxemia in children admitted for adenotonsillectomy .
	manualset3
91812	3	399278	13	NULL	NULL	0	NULL	 adenotonsillectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Identifying hypoxemia in children admitted for adenotonsillectomy .
	manualset3
91813	1	399279	13	NULL	NULL	0	NULL	intracellular targets	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Identifying the appropriate intracellular targets and understanding the signal transduction pathways in which these molecules participate are critical to this process .
	manualset3
91814	2	399279	13	NULL	NULL	0	NULL	signal transduction pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Identifying the appropriate intracellular targets and understanding the signal transduction pathways in which these molecules participate are critical to this process .
	manualset3
91815	3	399279	13	NULL	NULL	0	NULL	molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Identifying the appropriate intracellular targets and understanding the signal transduction pathways in which these molecules participate are critical to this process .
	manualset3
91816	4	399279	13	NULL	NULL	0	NULL	 process	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Identifying the appropriate intracellular targets and understanding the signal transduction pathways in which these molecules participate are critical to this process .
	manualset3
91817	1	399280	13	NULL	NULL	0	NULL	role 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Identifying the role of Refilins in organizing perinuclear actin networks provides additional insight in the process of intracellular mechanotransduction that regulate changes in cellular phenotype such as those observed during EMT .
	manualset3
91818	2	399280	13	NULL	NULL	0	NULL	Refilins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Identifying the role of Refilins in organizing perinuclear actin networks provides additional insight in the process of intracellular mechanotransduction that regulate changes in cellular phenotype such as those observed during EMT .
	manualset3
91823	3	399280	13	NULL	NULL	0	NULL	perinuclear actin networks 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Identifying the role of Refilins in organizing perinuclear actin networks provides additional insight in the process of intracellular mechanotransduction that regulate changes in cellular phenotype such as those observed during EMT .
	manualset3
91824	4	399280	13	NULL	NULL	0	NULL	process of intracellular mechanotransduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Identifying the role of Refilins in organizing perinuclear actin networks provides additional insight in the process of intracellular mechanotransduction that regulate changes in cellular phenotype such as those observed during EMT .
	manualset3
91826	5	399280	13	NULL	NULL	0	NULL	changes in cellular phenotype	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Identifying the role of Refilins in organizing perinuclear actin networks provides additional insight in the process of intracellular mechanotransduction that regulate changes in cellular phenotype such as those observed during EMT .
	manualset3
91827	6	399280	13	NULL	NULL	0	NULL	EMT	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Identifying the role of Refilins in organizing perinuclear actin networks provides additional insight in the process of intracellular mechanotransduction that regulate changes in cellular phenotype such as those observed during EMT .
	manualset3
91830	1	399281	13	NULL	NULL	0	NULL	Idiopathic intracranial hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Idiopathic intracranial hypertension and anticardolipin antibodies .
	manualset3
91832	2	399281	13	NULL	NULL	0	NULL	 anticardolipin antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Idiopathic intracranial hypertension and anticardolipin antibodies .
	manualset3
91834	1	399282	13	NULL	NULL	0	NULL	Idiopathic portal hypertension 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Idiopathic portal hypertension : a case report .
	manualset3
91836	2	399282	13	NULL	NULL	0	NULL	a case report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Idiopathic portal hypertension : a case report .
	manualset3
91839	1	399283	13	NULL	NULL	0	NULL	pathogenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If , as has been suggested , the pathogenesis of wound healing and tumor stroma generation is similar and dependent on fibrin deposition , then the types and amounts of fibrin deposited in wounds and tumors might also be expected to be similar .
	manualset3
91841	2	399283	13	NULL	NULL	0	NULL	wound healing 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If , as has been suggested , the pathogenesis of wound healing and tumor stroma generation is similar and dependent on fibrin deposition , then the types and amounts of fibrin deposited in wounds and tumors might also be expected to be similar .
	manualset3
91842	3	399283	13	NULL	NULL	0	NULL	tumor stroma generation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If , as has been suggested , the pathogenesis of wound healing and tumor stroma generation is similar and dependent on fibrin deposition , then the types and amounts of fibrin deposited in wounds and tumors might also be expected to be similar .
	manualset3
91843	4	399283	13	NULL	NULL	0	NULL	fibrin deposition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	If , as has been suggested , the pathogenesis of wound healing and tumor stroma generation is similar and dependent on fibrin deposition , then the types and amounts of fibrin deposited in wounds and tumors might also be expected to be similar .
	manualset3
91844	5	399283	13	NULL	NULL	0	NULL	types of fibrin	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	If , as has been suggested , the pathogenesis of wound healing and tumor stroma generation is similar and dependent on fibrin deposition , then the types and amounts of fibrin deposited in wounds and tumors might also be expected to be similar .
	manualset3
91845	6	399283	13	NULL	NULL	0	NULL	amounts of fibrin	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	If , as has been suggested , the pathogenesis of wound healing and tumor stroma generation is similar and dependent on fibrin deposition , then the types and amounts of fibrin deposited in wounds and tumors might also be expected to be similar .
	manualset3
91846	7	399283	13	NULL	NULL	0	NULL	wounds	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If , as has been suggested , the pathogenesis of wound healing and tumor stroma generation is similar and dependent on fibrin deposition , then the types and amounts of fibrin deposited in wounds and tumors might also be expected to be similar .
	manualset3
91847	8	399283	13	NULL	NULL	0	NULL	tumors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If , as has been suggested , the pathogenesis of wound healing and tumor stroma generation is similar and dependent on fibrin deposition , then the types and amounts of fibrin deposited in wounds and tumors might also be expected to be similar .
	manualset3
91848	1	399284	13	NULL	NULL	0	NULL	PIU	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	If PIU and these co-occurring disorders could be explained by shared risk factors or better as secondary disorders is largely unknown .
	manualset3
91849	2	399284	13	NULL	NULL	0	NULL	 disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If PIU and these co-occurring disorders could be explained by shared risk factors or better as secondary disorders is largely unknown .
	manualset3
91850	3	399284	13	NULL	NULL	0	NULL	risk factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If PIU and these co-occurring disorders could be explained by shared risk factors or better as secondary disorders is largely unknown .
	manualset3
91851	4	399284	13	NULL	NULL	0	NULL	secondary disorders 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If PIU and these co-occurring disorders could be explained by shared risk factors or better as secondary disorders is largely unknown .
	manualset3
91852	1	399285	13	NULL	NULL	0	NULL	male 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	If a male has a paternity of less than unity , then another male or other males must have gained the lost paternity .
	manualset3
91855	2	399285	13	NULL	NULL	0	NULL	paternity of less than unity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	If a male has a paternity of less than unity , then another male or other males must have gained the lost paternity .
	manualset3
91856	3	399285	13	NULL	NULL	0	NULL	male 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	If a male has a paternity of less than unity , then another male or other males must have gained the lost paternity .
	manualset3
91857	4	399285	13	NULL	NULL	0	NULL	males	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	If a male has a paternity of less than unity , then another male or other males must have gained the lost paternity .
	manualset3
91860	5	399285	13	NULL	NULL	0	NULL	paternity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	If a male has a paternity of less than unity , then another male or other males must have gained the lost paternity .
	manualset3
91861	1	399286	13	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	If a patient is predicted to derive little advantage from chemotherapy in the adjuvant setting , it is equally unlikely that an advantage will be seen with neoadjuvant chemotherapy .
	manualset3
91863	2	399286	13	NULL	NULL	0	NULL	 chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	If a patient is predicted to derive little advantage from chemotherapy in the adjuvant setting , it is equally unlikely that an advantage will be seen with neoadjuvant chemotherapy .
	manualset3
91864	3	399286	13	NULL	NULL	0	NULL	adjuvant setting	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	If a patient is predicted to derive little advantage from chemotherapy in the adjuvant setting , it is equally unlikely that an advantage will be seen with neoadjuvant chemotherapy .
	manualset3
91865	4	399286	13	NULL	NULL	0	NULL	neoadjuvant chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	If a patient is predicted to derive little advantage from chemotherapy in the adjuvant setting , it is equally unlikely that an advantage will be seen with neoadjuvant chemotherapy .
	manualset3
91867	5	399286	13	NULL	NULL	0	NULL	advantage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If a patient is predicted to derive little advantage from chemotherapy in the adjuvant setting , it is equally unlikely that an advantage will be seen with neoadjuvant chemotherapy .
	manualset3
91868	6	399286	13	NULL	NULL	0	NULL	 advantage 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If a patient is predicted to derive little advantage from chemotherapy in the adjuvant setting , it is equally unlikely that an advantage will be seen with neoadjuvant chemotherapy .
	manualset3
91869	1	399287	13	NULL	NULL	0	NULL	working diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	If a working diagnosis of congestive heart failure was made only on the basis of the most common probability , and the fluid supply was restricted , HHNKDC would readily occur or be aggravated by the dehydration iatrogenically produced .
	manualset3
91870	2	399287	13	NULL	NULL	0	NULL	 congestive heart failure 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If a working diagnosis of congestive heart failure was made only on the basis of the most common probability , and the fluid supply was restricted , HHNKDC would readily occur or be aggravated by the dehydration iatrogenically produced .
	manualset3
91871	3	399287	13	NULL	NULL	0	NULL	common probability	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	If a working diagnosis of congestive heart failure was made only on the basis of the most common probability , and the fluid supply was restricted , HHNKDC would readily occur or be aggravated by the dehydration iatrogenically produced .
	manualset3
91872	4	399287	13	NULL	NULL	NULL	NULL	fluid 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	If a working diagnosis of congestive heart failure was made only on the basis of the most common probability , and the fluid supply was restricted , HHNKDC would readily occur or be aggravated by the dehydration iatrogenically produced .
	manualset3
91873	5	399287	13	NULL	NULL	0	NULL	HHNKDC 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If a working diagnosis of congestive heart failure was made only on the basis of the most common probability , and the fluid supply was restricted , HHNKDC would readily occur or be aggravated by the dehydration iatrogenically produced .
	manualset3
91874	6	399287	13	NULL	NULL	0	NULL	dehydration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If a working diagnosis of congestive heart failure was made only on the basis of the most common probability , and the fluid supply was restricted , HHNKDC would readily occur or be aggravated by the dehydration iatrogenically produced .
	manualset3
91875	1	399288	13	NULL	NULL	0	NULL	 interferometer	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	If an interferometer is available for quantitative wave-front analysis on the production line , the point-spread function may quite easily be computed from an interferogram of the wave front in the back focal plane of a micro-objective .
	manualset3
91877	2	399288	13	NULL	NULL	0	NULL	quantitative wave-front analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	If an interferometer is available for quantitative wave-front analysis on the production line , the point-spread function may quite easily be computed from an interferogram of the wave front in the back focal plane of a micro-objective .
	manualset3
91895	3	399288	13	NULL	NULL	0	NULL	production line 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	If an interferometer is available for quantitative wave-front analysis on the production line , the point-spread function may quite easily be computed from an interferogram of the wave front in the back focal plane of a micro-objective .
	manualset3
91896	4	399288	13	NULL	NULL	0	NULL	point-spread function 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	If an interferometer is available for quantitative wave-front analysis on the production line , the point-spread function may quite easily be computed from an interferogram of the wave front in the back focal plane of a micro-objective .
	manualset3
91897	5	399288	13	NULL	NULL	0	NULL	interferogram of the wave front 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	If an interferometer is available for quantitative wave-front analysis on the production line , the point-spread function may quite easily be computed from an interferogram of the wave front in the back focal plane of a micro-objective .
	manualset3
91898	6	399288	13	NULL	NULL	0	NULL	back focal plane 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	If an interferometer is available for quantitative wave-front analysis on the production line , the point-spread function may quite easily be computed from an interferogram of the wave front in the back focal plane of a micro-objective .
	manualset3
91899	7	399288	13	NULL	NULL	0	NULL	micro-objective	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	If an interferometer is available for quantitative wave-front analysis on the production line , the point-spread function may quite easily be computed from an interferogram of the wave front in the back focal plane of a micro-objective .
	manualset3
91900	1	399289	13	NULL	NULL	0	NULL	bladder cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	If bladder cancer is caused by agents present in the urine , as is widely believed , this mechanism may also protect against carcinogenesis .
	manualset3
91901	2	399289	13	NULL	NULL	0	NULL	 agents	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	If bladder cancer is caused by agents present in the urine , as is widely believed , this mechanism may also protect against carcinogenesis .
	manualset3
91902	3	399289	13	NULL	NULL	0	NULL	urine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	If bladder cancer is caused by agents present in the urine , as is widely believed , this mechanism may also protect against carcinogenesis .
	manualset3
91903	4	399289	13	NULL	NULL	0	NULL	mechanism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	If bladder cancer is caused by agents present in the urine , as is widely believed , this mechanism may also protect against carcinogenesis .
	manualset3
91904	5	399289	13	NULL	NULL	0	NULL	 carcinogenesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	If bladder cancer is caused by agents present in the urine , as is widely believed , this mechanism may also protect against carcinogenesis .
	manualset3
91905	1	399290	13	NULL	NULL	0	NULL	combination therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	If combination therapy with OAD is not successful in achieving HbA1c values & lt ; 6.5 % , insulin therapy is required either in combination with OADs as a bedtime regimen or as intensive insulin therapy using both basal and short-term acting insulins .
	manualset3
91906	2	399290	13	NULL	NULL	0	NULL	OAD 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	If combination therapy with OAD is not successful in achieving HbA1c values & lt ; 6.5 % , insulin therapy is required either in combination with OADs as a bedtime regimen or as intensive insulin therapy using both basal and short-term acting insulins .
	manualset3
91907	3	399290	13	NULL	NULL	0	NULL	HbA1c values	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If combination therapy with OAD is not successful in achieving HbA1c values & lt ; 6.5 % , insulin therapy is required either in combination with OADs as a bedtime regimen or as intensive insulin therapy using both basal and short-term acting insulins .
	manualset3
91908	4	399290	13	NULL	NULL	0	NULL	6.5 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	If combination therapy with OAD is not successful in achieving HbA1c values & lt ; 6.5 % , insulin therapy is required either in combination with OADs as a bedtime regimen or as intensive insulin therapy using both basal and short-term acting insulins .
	manualset3
91909	5	399290	13	NULL	NULL	0	NULL	 insulin therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	If combination therapy with OAD is not successful in achieving HbA1c values & lt ; 6.5 % , insulin therapy is required either in combination with OADs as a bedtime regimen or as intensive insulin therapy using both basal and short-term acting insulins .
	manualset3
91910	6	399290	13	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	If combination therapy with OAD is not successful in achieving HbA1c values & lt ; 6.5 % , insulin therapy is required either in combination with OADs as a bedtime regimen or as intensive insulin therapy using both basal and short-term acting insulins .
	manualset3
91911	7	399290	13	NULL	NULL	0	NULL	OADs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	If combination therapy with OAD is not successful in achieving HbA1c values & lt ; 6.5 % , insulin therapy is required either in combination with OADs as a bedtime regimen or as intensive insulin therapy using both basal and short-term acting insulins .
	manualset3
91912	8	399290	13	NULL	NULL	0	NULL	bedtime regimen	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	If combination therapy with OAD is not successful in achieving HbA1c values & lt ; 6.5 % , insulin therapy is required either in combination with OADs as a bedtime regimen or as intensive insulin therapy using both basal and short-term acting insulins .
	manualset3
91913	9	399290	13	NULL	NULL	0	NULL	intensive insulin therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	If combination therapy with OAD is not successful in achieving HbA1c values & lt ; 6.5 % , insulin therapy is required either in combination with OADs as a bedtime regimen or as intensive insulin therapy using both basal and short-term acting insulins .
	manualset3
91914	10	399290	13	NULL	NULL	NULL	NULL	 insulins 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	If combination therapy with OAD is not successful in achieving HbA1c values & lt ; 6.5 % , insulin therapy is required either in combination with OADs as a bedtime regimen or as intensive insulin therapy using both basal and short-term acting insulins .
	manualset3
91915	1	399291	13	NULL	NULL	0	NULL	delivery modules	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	If developed , delivery modules would bring targeting molecules across the BBB to their respective active sites .
	manualset3
91916	2	399291	13	NULL	NULL	0	NULL	targeting molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	If developed , delivery modules would bring targeting molecules across the BBB to their respective active sites .
	manualset3
91917	3	399291	13	NULL	NULL	NULL	NULL	BBB	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	If developed , delivery modules would bring targeting molecules across the BBB to their respective active sites .
	manualset3
91918	4	399291	13	NULL	NULL	0	NULL	active sites 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	If developed , delivery modules would bring targeting molecules across the BBB to their respective active sites .
	manualset3
91919	1	399292	13	NULL	NULL	0	NULL	heparanase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	If heparanase is the answer , what is the question ?
	manualset3
91920	2	399292	13	NULL	NULL	0	NULL	answer 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	If heparanase is the answer , what is the question ?
	manualset3
91921	3	399292	13	NULL	NULL	0	NULL	question	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	If heparanase is the answer , what is the question ?
	manualset3
91922	1	399293	13	NULL	NULL	0	NULL	stapedius reflex 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( The use of the stapedius reflex in the fitting of hearing aids ( author transl ) ) .
	manualset3
91923	2	399293	13	NULL	NULL	0	NULL	hearing aids 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( The use of the stapedius reflex in the fitting of hearing aids ( author transl ) ) .
	manualset3
91924	3	399293	13	NULL	NULL	0	NULL	author	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( The use of the stapedius reflex in the fitting of hearing aids ( author transl ) ) .
	manualset3
91926	1	399294	13	NULL	NULL	0	NULL	perceptual phenomenon	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	If it is agreed that this perceptual phenomenon is causally linked to the activity of nerve cells , the state jumps would have to occur in conjunction with changes in neural activity somewhere in the nervous system .
	manualset3
91927	2	399294	13	NULL	NULL	0	NULL	activity of nerve cells	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	If it is agreed that this perceptual phenomenon is causally linked to the activity of nerve cells , the state jumps would have to occur in conjunction with changes in neural activity somewhere in the nervous system .
	manualset3
91929	3	399294	13	NULL	NULL	0	NULL	conjunction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	If it is agreed that this perceptual phenomenon is causally linked to the activity of nerve cells , the state jumps would have to occur in conjunction with changes in neural activity somewhere in the nervous system .
	manualset3
91931	4	399294	13	NULL	NULL	0	NULL	neural activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	If it is agreed that this perceptual phenomenon is causally linked to the activity of nerve cells , the state jumps would have to occur in conjunction with changes in neural activity somewhere in the nervous system .
	manualset3
91932	5	399294	13	NULL	NULL	0	NULL	nervous system 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	If it is agreed that this perceptual phenomenon is causally linked to the activity of nerve cells , the state jumps would have to occur in conjunction with changes in neural activity somewhere in the nervous system .
	manualset3
91933	1	399295	13	NULL	NULL	0	NULL	hair 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	If it were possible to pool all hair belonging to an individual prior to DNA analysis , then this effort could not only be reduced , but the number of hair for an STR-approach could also be increased .
	manualset3
91934	2	399295	13	NULL	NULL	0	NULL	individual	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	If it were possible to pool all hair belonging to an individual prior to DNA analysis , then this effort could not only be reduced , but the number of hair for an STR-approach could also be increased .
	manualset3
91935	3	399295	13	NULL	NULL	0	NULL	prior to DNA analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	If it were possible to pool all hair belonging to an individual prior to DNA analysis , then this effort could not only be reduced , but the number of hair for an STR-approach could also be increased .
	manualset3
91936	4	399295	13	NULL	NULL	0	NULL	effort 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	If it were possible to pool all hair belonging to an individual prior to DNA analysis , then this effort could not only be reduced , but the number of hair for an STR-approach could also be increased .
	manualset3
91937	5	399295	13	NULL	NULL	0	NULL	number of hair	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	If it were possible to pool all hair belonging to an individual prior to DNA analysis , then this effort could not only be reduced , but the number of hair for an STR-approach could also be increased .
	manualset3
91938	6	399295	13	NULL	NULL	0	NULL	STR-approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	If it were possible to pool all hair belonging to an individual prior to DNA analysis , then this effort could not only be reduced , but the number of hair for an STR-approach could also be increased .
	manualset3
91939	1	399296	13	NULL	NULL	0	NULL	 left portal ducts 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	If left portal ducts are inaccessible by division of the main portal fissure because of a retroportal location , then an anastomosis in the anterior portion of the umbilical fissure may give adequate drainage .
	manualset3
91940	2	399296	13	NULL	NULL	0	NULL	division	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	If left portal ducts are inaccessible by division of the main portal fissure because of a retroportal location , then an anastomosis in the anterior portion of the umbilical fissure may give adequate drainage .
	manualset3
91941	3	399296	13	NULL	NULL	0	NULL	main portal fissure 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	If left portal ducts are inaccessible by division of the main portal fissure because of a retroportal location , then an anastomosis in the anterior portion of the umbilical fissure may give adequate drainage .
	manualset3
91942	4	399296	13	NULL	NULL	0	NULL	retroportal location	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	If left portal ducts are inaccessible by division of the main portal fissure because of a retroportal location , then an anastomosis in the anterior portion of the umbilical fissure may give adequate drainage .
	manualset3
91943	5	399296	13	NULL	NULL	0	NULL	 anastomosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	If left portal ducts are inaccessible by division of the main portal fissure because of a retroportal location , then an anastomosis in the anterior portion of the umbilical fissure may give adequate drainage .
	manualset3
91944	6	399296	13	NULL	NULL	0	NULL	anterior portion of the umbilical fissure	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	If left portal ducts are inaccessible by division of the main portal fissure because of a retroportal location , then an anastomosis in the anterior portion of the umbilical fissure may give adequate drainage .
	manualset3
91945	7	399296	13	NULL	NULL	0	NULL	adequate drainage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	If left portal ducts are inaccessible by division of the main portal fissure because of a retroportal location , then an anastomosis in the anterior portion of the umbilical fissure may give adequate drainage .
	manualset3
91946	1	399297	13	NULL	NULL	0	NULL	metal chloride 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	If metal chloride or nitrate salts are used in the reaction with the LDH then co-intercalation of either the Cl ( - ) or NO ( 3 ) ( - ) anions is observed .
	manualset3
91947	2	399297	13	NULL	NULL	0	NULL	 nitrate salts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	If metal chloride or nitrate salts are used in the reaction with the LDH then co-intercalation of either the Cl ( - ) or NO ( 3 ) ( - ) anions is observed .
	manualset3
91948	3	399297	13	NULL	NULL	0	NULL	reaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	If metal chloride or nitrate salts are used in the reaction with the LDH then co-intercalation of either the Cl ( - ) or NO ( 3 ) ( - ) anions is observed .
	manualset3
91949	4	399297	13	NULL	NULL	0	NULL	LDH	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	If metal chloride or nitrate salts are used in the reaction with the LDH then co-intercalation of either the Cl ( - ) or NO ( 3 ) ( - ) anions is observed .
	manualset3
91950	5	399297	13	NULL	NULL	0	NULL	co-intercalation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	If metal chloride or nitrate salts are used in the reaction with the LDH then co-intercalation of either the Cl ( - ) or NO ( 3 ) ( - ) anions is observed .
	manualset3
91951	6	399297	13	NULL	NULL	0	NULL	Cl ( - )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	If metal chloride or nitrate salts are used in the reaction with the LDH then co-intercalation of either the Cl ( - ) or NO ( 3 ) ( - ) anions is observed .
	manualset3
91952	7	399297	13	NULL	NULL	0	NULL	NO ( 3 ) ( - ) anions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	If metal chloride or nitrate salts are used in the reaction with the LDH then co-intercalation of either the Cl ( - ) or NO ( 3 ) ( - ) anions is observed .
	manualset3
91959	1	399298	13	NULL	NULL	0	NULL	GVHD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	If more effective control of GVHD can be accomplished , marrow transplantation between MLC-reactive individuals may become feasible .
	manualset3
91960	2	399298	13	NULL	NULL	0	NULL	marrow transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	If more effective control of GVHD can be accomplished , marrow transplantation between MLC-reactive individuals may become feasible .
	manualset3
91961	3	399298	13	NULL	NULL	0	NULL	MLC-reactive individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	If more effective control of GVHD can be accomplished , marrow transplantation between MLC-reactive individuals may become feasible .
	manualset3
91964	1	399299	13	NULL	NULL	0	NULL	energy	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	If most of the energy of the inconsistencies is limited to a certain region of kappa-space , increased sampling density ( oversampling ) in this region can be especially effective in reducing motion artifacts .
	manualset3
91965	2	399299	13	NULL	NULL	0	NULL	inconsistencies 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	If most of the energy of the inconsistencies is limited to a certain region of kappa-space , increased sampling density ( oversampling ) in this region can be especially effective in reducing motion artifacts .
	manualset3
91966	3	399299	13	NULL	NULL	NULL	NULL	certain region of kappa-space	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	If most of the energy of the inconsistencies is limited to a certain region of kappa-space , increased sampling density ( oversampling ) in this region can be especially effective in reducing motion artifacts .
	manualset3
91967	4	399299	13	NULL	NULL	0	NULL	sampling density ( oversampling )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	If most of the energy of the inconsistencies is limited to a certain region of kappa-space , increased sampling density ( oversampling ) in this region can be especially effective in reducing motion artifacts .
	manualset3
91968	5	399299	13	NULL	NULL	0	NULL	reducing motion artifacts 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	If most of the energy of the inconsistencies is limited to a certain region of kappa-space , increased sampling density ( oversampling ) in this region can be especially effective in reducing motion artifacts .
	manualset3
91969	1	399300	13	NULL	NULL	NULL	NULL	agents 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	If recent results consistently show the superiority of these agents over tamoxifen , the therapeutic strategies of AIs in adjuvant setting are still debated .
	manualset3
91970	2	399300	13	NULL	NULL	0	NULL	 tamoxifen	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	If recent results consistently show the superiority of these agents over tamoxifen , the therapeutic strategies of AIs in adjuvant setting are still debated .
	manualset3
91971	3	399300	13	NULL	NULL	0	NULL	therapeutic strategies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	If recent results consistently show the superiority of these agents over tamoxifen , the therapeutic strategies of AIs in adjuvant setting are still debated .
	manualset3
91972	4	399300	13	NULL	NULL	0	NULL	AIs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	If recent results consistently show the superiority of these agents over tamoxifen , the therapeutic strategies of AIs in adjuvant setting are still debated .
	manualset3
91973	5	399300	13	NULL	NULL	0	NULL	adjuvant setting	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	If recent results consistently show the superiority of these agents over tamoxifen , the therapeutic strategies of AIs in adjuvant setting are still debated .
	manualset3
91974	1	399301	13	NULL	NULL	0	NULL	salt fluoridation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	If salt fluoridation could also be generalized , caries levels could be reduced to a fraction of their initial values .
	manualset3
91975	2	399301	13	NULL	NULL	0	NULL	 caries levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If salt fluoridation could also be generalized , caries levels could be reduced to a fraction of their initial values .
	manualset3
91976	3	399301	13	NULL	NULL	0	NULL	fraction of their initial values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	If salt fluoridation could also be generalized , caries levels could be reduced to a fraction of their initial values .
	manualset3
91977	1	399302	13	NULL	NULL	0	NULL	hip 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	If screened only at the hip or spine , 17.9 / 27.3 % with osteopenia and 1.3 / 2.9 % with osteoporosis at either site would be diagnosed as normal .
	manualset3
91978	2	399302	13	NULL	NULL	0	NULL	 spine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	If screened only at the hip or spine , 17.9 / 27.3 % with osteopenia and 1.3 / 2.9 % with osteoporosis at either site would be diagnosed as normal .
	manualset3
91979	3	399302	13	NULL	NULL	0	NULL	 17.9 / 27.3 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	If screened only at the hip or spine , 17.9 / 27.3 % with osteopenia and 1.3 / 2.9 % with osteoporosis at either site would be diagnosed as normal .
	manualset3
91980	4	399302	13	NULL	NULL	0	NULL	osteopenia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If screened only at the hip or spine , 17.9 / 27.3 % with osteopenia and 1.3 / 2.9 % with osteoporosis at either site would be diagnosed as normal .
	manualset3
91981	5	399302	13	NULL	NULL	0	NULL	1.3 / 2.9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	If screened only at the hip or spine , 17.9 / 27.3 % with osteopenia and 1.3 / 2.9 % with osteoporosis at either site would be diagnosed as normal .
	manualset3
91982	6	399302	13	NULL	NULL	0	NULL	osteoporosis at either site	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If screened only at the hip or spine , 17.9 / 27.3 % with osteopenia and 1.3 / 2.9 % with osteoporosis at either site would be diagnosed as normal .
	manualset3
91983	1	399303	13	NULL	NULL	0	NULL	value of CT	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( The value of CT in the differential diagnostic evaluation of masses in the left upper abdominal quadrant ( author 's transl ) ) .
	manualset3
91984	2	399303	13	NULL	NULL	0	NULL	differential diagnostic evaluation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( The value of CT in the differential diagnostic evaluation of masses in the left upper abdominal quadrant ( author 's transl ) ) .
	manualset3
91985	3	399303	13	NULL	NULL	0	NULL	masses in the left upper abdominal quadrant 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( The value of CT in the differential diagnostic evaluation of masses in the left upper abdominal quadrant ( author 's transl ) ) .
	manualset3
91986	4	399303	13	NULL	NULL	0	NULL	author 's	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( The value of CT in the differential diagnostic evaluation of masses in the left upper abdominal quadrant ( author 's transl ) ) .
	manualset3
91988	2	399304	13	NULL	NULL	0	NULL	nitric oxide donors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	If so , it will be interesting to study whether nitric oxide donors and/or nitric oxide precursors can be given together with estrogen , statins , or essential fatty acids to potentiate their benefit in osteoporosis .
	manualset3
91989	3	399304	13	NULL	NULL	0	NULL	nitric oxide precursors 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	If so , it will be interesting to study whether nitric oxide donors and/or nitric oxide precursors can be given together with estrogen , statins , or essential fatty acids to potentiate their benefit in osteoporosis .
	manualset3
91990	4	399304	13	NULL	NULL	0	NULL	estrogen 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	If so , it will be interesting to study whether nitric oxide donors and/or nitric oxide precursors can be given together with estrogen , statins , or essential fatty acids to potentiate their benefit in osteoporosis .
	manualset3
91991	5	399304	13	NULL	NULL	0	NULL	statins	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	If so , it will be interesting to study whether nitric oxide donors and/or nitric oxide precursors can be given together with estrogen , statins , or essential fatty acids to potentiate their benefit in osteoporosis .
	manualset3
91992	6	399304	13	NULL	NULL	0	NULL	essential fatty acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	If so , it will be interesting to study whether nitric oxide donors and/or nitric oxide precursors can be given together with estrogen , statins , or essential fatty acids to potentiate their benefit in osteoporosis .
	manualset3
91993	7	399304	13	NULL	NULL	0	NULL	osteoporosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If so , it will be interesting to study whether nitric oxide donors and/or nitric oxide precursors can be given together with estrogen , statins , or essential fatty acids to potentiate their benefit in osteoporosis .
	manualset3
91994	1	399305	13	NULL	NULL	0	NULL	crustal extraction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	If so , such crustal extraction should have left a chemical fingerprint in the isotopic composition of the mantle .
	manualset3
91995	2	399305	13	NULL	NULL	0	NULL	 chemical fingerprint 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	If so , such crustal extraction should have left a chemical fingerprint in the isotopic composition of the mantle .
	manualset3
91996	3	399305	13	NULL	NULL	0	NULL	isotopic composition	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	If so , such crustal extraction should have left a chemical fingerprint in the isotopic composition of the mantle .
	manualset3
91997	4	399305	13	NULL	NULL	0	NULL	mantle	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	If so , such crustal extraction should have left a chemical fingerprint in the isotopic composition of the mantle .
	manualset3
91998	1	399306	13	NULL	NULL	0	NULL	chest picture 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	If the chest picture is abnormal , further investigations will be required and , according to the results , preventive treatment or polychemotherapy for tuberculosis disease will be administered .
	manualset3
91999	2	399306	13	NULL	NULL	0	NULL	investigations 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	If the chest picture is abnormal , further investigations will be required and , according to the results , preventive treatment or polychemotherapy for tuberculosis disease will be administered .
	manualset3
92000	3	399306	13	NULL	NULL	0	NULL	preventive treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	If the chest picture is abnormal , further investigations will be required and , according to the results , preventive treatment or polychemotherapy for tuberculosis disease will be administered .
	manualset3
92001	4	399306	13	NULL	NULL	0	NULL	polychemotherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	If the chest picture is abnormal , further investigations will be required and , according to the results , preventive treatment or polychemotherapy for tuberculosis disease will be administered .
	manualset3
92002	5	399306	13	NULL	NULL	0	NULL	tuberculosis disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	If the chest picture is abnormal , further investigations will be required and , according to the results , preventive treatment or polychemotherapy for tuberculosis disease will be administered .
	manualset3
92003	1	399307	13	NULL	NULL	0	NULL	fiber	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	If the fiber and obstacle only interact via excluded volume , there are small corrections to the Brownian ratchet predictions which suggest that tip fluctuations play a minor role .
	manualset3
92004	2	399307	13	NULL	NULL	0	NULL	obstacle 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	If the fiber and obstacle only interact via excluded volume , there are small corrections to the Brownian ratchet predictions which suggest that tip fluctuations play a minor role .
	manualset3
92005	3	399307	13	NULL	NULL	0	NULL	volume	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	If the fiber and obstacle only interact via excluded volume , there are small corrections to the Brownian ratchet predictions which suggest that tip fluctuations play a minor role .
	manualset3
92006	4	399307	13	NULL	NULL	0	NULL	corrections	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	If the fiber and obstacle only interact via excluded volume , there are small corrections to the Brownian ratchet predictions which suggest that tip fluctuations play a minor role .
	manualset3
92007	5	399307	13	NULL	NULL	0	NULL	 Brownian ratchet predictions	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	If the fiber and obstacle only interact via excluded volume , there are small corrections to the Brownian ratchet predictions which suggest that tip fluctuations play a minor role .
	manualset3
92008	6	399307	13	NULL	NULL	0	NULL	tip fluctuations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	If the fiber and obstacle only interact via excluded volume , there are small corrections to the Brownian ratchet predictions which suggest that tip fluctuations play a minor role .
	manualset3
92009	1	399308	13	NULL	NULL	0	NULL	gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	If the gene encodes a protein that is closely related to known proteins , gene identification is aided by matching similarity of potential translation products to those target proteins .
	manualset3
92010	2	399308	13	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	If the gene encodes a protein that is closely related to known proteins , gene identification is aided by matching similarity of potential translation products to those target proteins .
	manualset3
92011	3	399308	13	NULL	NULL	0	NULL	proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	If the gene encodes a protein that is closely related to known proteins , gene identification is aided by matching similarity of potential translation products to those target proteins .
	manualset3
92012	4	399308	13	NULL	NULL	0	NULL	gene identification 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	If the gene encodes a protein that is closely related to known proteins , gene identification is aided by matching similarity of potential translation products to those target proteins .
	manualset3
92013	5	399308	13	NULL	NULL	0	NULL	similarity	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	If the gene encodes a protein that is closely related to known proteins , gene identification is aided by matching similarity of potential translation products to those target proteins .
	manualset3
92014	6	399308	13	NULL	NULL	0	NULL	potential translation products 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	If the gene encodes a protein that is closely related to known proteins , gene identification is aided by matching similarity of potential translation products to those target proteins .
	manualset3
92015	7	399308	13	NULL	NULL	0	NULL	target proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	If the gene encodes a protein that is closely related to known proteins , gene identification is aided by matching similarity of potential translation products to those target proteins .
	manualset3
92016	1	399309	13	NULL	NULL	0	NULL	 pre-ablation bridging strategy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	If the latter approach is chosen , a pre-ablation bridging strategy of enoxaparin 1mg/kg twice daily is reasonable in selected patients unless the patient 's bleeding risk dictates using a lower dose regimen ( 0.5 mg/kg twice daily ) or avoiding bridging altogether .
	manualset3
92017	2	399309	13	NULL	NULL	0	NULL	enoxaparin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	If the latter approach is chosen , a pre-ablation bridging strategy of enoxaparin 1mg/kg twice daily is reasonable in selected patients unless the patient 's bleeding risk dictates using a lower dose regimen ( 0.5 mg/kg twice daily ) or avoiding bridging altogether .
	manualset3
92018	3	399309	13	NULL	NULL	0	NULL	1mg/kg twice daily	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	If the latter approach is chosen , a pre-ablation bridging strategy of enoxaparin 1mg/kg twice daily is reasonable in selected patients unless the patient 's bleeding risk dictates using a lower dose regimen ( 0.5 mg/kg twice daily ) or avoiding bridging altogether .
	manualset3
92019	4	399309	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	If the latter approach is chosen , a pre-ablation bridging strategy of enoxaparin 1mg/kg twice daily is reasonable in selected patients unless the patient 's bleeding risk dictates using a lower dose regimen ( 0.5 mg/kg twice daily ) or avoiding bridging altogether .
	manualset3
92020	5	399309	13	NULL	NULL	0	NULL	patient 's	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	If the latter approach is chosen , a pre-ablation bridging strategy of enoxaparin 1mg/kg twice daily is reasonable in selected patients unless the patient 's bleeding risk dictates using a lower dose regimen ( 0.5 mg/kg twice daily ) or avoiding bridging altogether .
	manualset3
92021	6	399309	13	NULL	NULL	0	NULL	bleeding risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If the latter approach is chosen , a pre-ablation bridging strategy of enoxaparin 1mg/kg twice daily is reasonable in selected patients unless the patient 's bleeding risk dictates using a lower dose regimen ( 0.5 mg/kg twice daily ) or avoiding bridging altogether .
	manualset3
92022	7	399309	13	NULL	NULL	0	NULL	lower dose regimen	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	If the latter approach is chosen , a pre-ablation bridging strategy of enoxaparin 1mg/kg twice daily is reasonable in selected patients unless the patient 's bleeding risk dictates using a lower dose regimen ( 0.5 mg/kg twice daily ) or avoiding bridging altogether .
	manualset3
92023	8	399309	13	NULL	NULL	0	NULL	0.5 mg/kg twice daily	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	If the latter approach is chosen , a pre-ablation bridging strategy of enoxaparin 1mg/kg twice daily is reasonable in selected patients unless the patient 's bleeding risk dictates using a lower dose regimen ( 0.5 mg/kg twice daily ) or avoiding bridging altogether .
	manualset3
92024	1	399310	13	NULL	NULL	0	NULL	 leachate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	If the leachate continues to migrate at this apparent rate , it will take more than 100 years to reach the water table .
	manualset3
92025	2	399310	13	NULL	NULL	0	NULL	apparent rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	If the leachate continues to migrate at this apparent rate , it will take more than 100 years to reach the water table .
	manualset3
92026	3	399310	13	NULL	NULL	0	NULL	100 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	If the leachate continues to migrate at this apparent rate , it will take more than 100 years to reach the water table .
	manualset3
92027	4	399310	13	NULL	NULL	0	NULL	water table	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	If the leachate continues to migrate at this apparent rate , it will take more than 100 years to reach the water table .
	manualset3
92028	1	399311	13	NULL	NULL	0	NULL	neoplastic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	If the neoplastic cells on slides are mixed with nonneoplastic lymphocytes , cells of interest are isolated by microdissection .
	manualset3
92029	2	399311	13	NULL	NULL	0	NULL	slides	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	If the neoplastic cells on slides are mixed with nonneoplastic lymphocytes , cells of interest are isolated by microdissection .
	manualset3
92030	3	399311	13	NULL	NULL	0	NULL	nonneoplastic lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	If the neoplastic cells on slides are mixed with nonneoplastic lymphocytes , cells of interest are isolated by microdissection .
	manualset3
92031	4	399311	13	NULL	NULL	0	NULL	cells of interest	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	If the neoplastic cells on slides are mixed with nonneoplastic lymphocytes , cells of interest are isolated by microdissection .
	manualset3
92032	5	399311	13	NULL	NULL	0	NULL	microdissection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	If the neoplastic cells on slides are mixed with nonneoplastic lymphocytes , cells of interest are isolated by microdissection .
	manualset3
92033	1	399312	13	NULL	NULL	0	NULL	patient 's condition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If the patient 's condition permits , it may be useful to opacify the dilated segment in order to study the nature of the obstacle .
	manualset3
92034	2	399312	13	NULL	NULL	0	NULL	dilated segment	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	If the patient 's condition permits , it may be useful to opacify the dilated segment in order to study the nature of the obstacle .
	manualset3
92035	3	399312	13	NULL	NULL	0	NULL	nature of the obstacle	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If the patient 's condition permits , it may be useful to opacify the dilated segment in order to study the nature of the obstacle .
	manualset3
92036	1	399313	13	NULL	NULL	0	NULL	value 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( The value of MRI for diagnosis of recurrence of rectal carcinoma after surgical resection ) .
	manualset3
92037	2	399313	13	NULL	NULL	0	NULL	MRI	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( The value of MRI for diagnosis of recurrence of rectal carcinoma after surgical resection ) .
	manualset3
92038	3	399313	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( The value of MRI for diagnosis of recurrence of rectal carcinoma after surgical resection ) .
	manualset3
92039	4	399313	13	NULL	NULL	NULL	NULL	recurrence of rectal carcinoma	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The value of MRI for diagnosis of recurrence of rectal carcinoma after surgical resection ) .
	manualset3
92040	5	399313	13	NULL	NULL	0	NULL	surgical resection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( The value of MRI for diagnosis of recurrence of rectal carcinoma after surgical resection ) .
	manualset3
92041	1	399314	13	NULL	NULL	0	NULL	 time span 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	If the time span of risk of perinatal death is defined as the period from 20 weeks gestation through 27 days after birth , 97 out of 100 infants born in California during 1959 were born alive and survived the first month of life .
	manualset3
92042	2	399314	13	NULL	NULL	0	NULL	risk of perinatal death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If the time span of risk of perinatal death is defined as the period from 20 weeks gestation through 27 days after birth , 97 out of 100 infants born in California during 1959 were born alive and survived the first month of life .
	manualset3
92043	3	399314	13	NULL	NULL	0	NULL	period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	If the time span of risk of perinatal death is defined as the period from 20 weeks gestation through 27 days after birth , 97 out of 100 infants born in California during 1959 were born alive and survived the first month of life .
	manualset3
92044	4	399314	13	NULL	NULL	0	NULL	20 weeks gestation through 27 days after birth	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	If the time span of risk of perinatal death is defined as the period from 20 weeks gestation through 27 days after birth , 97 out of 100 infants born in California during 1959 were born alive and survived the first month of life .
	manualset3
92045	5	399314	13	NULL	NULL	0	NULL	97 out of 100	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	If the time span of risk of perinatal death is defined as the period from 20 weeks gestation through 27 days after birth , 97 out of 100 infants born in California during 1959 were born alive and survived the first month of life .
	manualset3
92046	6	399314	13	NULL	NULL	0	NULL	infants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	If the time span of risk of perinatal death is defined as the period from 20 weeks gestation through 27 days after birth , 97 out of 100 infants born in California during 1959 were born alive and survived the first month of life .
	manualset3
92047	7	399314	13	NULL	NULL	0	NULL	California	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	If the time span of risk of perinatal death is defined as the period from 20 weeks gestation through 27 days after birth , 97 out of 100 infants born in California during 1959 were born alive and survived the first month of life .
	manualset3
92048	8	399314	13	NULL	NULL	0	NULL	1959 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	If the time span of risk of perinatal death is defined as the period from 20 weeks gestation through 27 days after birth , 97 out of 100 infants born in California during 1959 were born alive and survived the first month of life .
	manualset3
92049	9	399314	13	NULL	NULL	0	NULL	alive	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If the time span of risk of perinatal death is defined as the period from 20 weeks gestation through 27 days after birth , 97 out of 100 infants born in California during 1959 were born alive and survived the first month of life .
	manualset3
92050	10	399314	13	NULL	NULL	0	NULL	first month of life	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	If the time span of risk of perinatal death is defined as the period from 20 weeks gestation through 27 days after birth , 97 out of 100 infants born in California during 1959 were born alive and survived the first month of life .
	manualset3
92051	1	399315	13	NULL	NULL	0	NULL	factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If these factors are absent , another chronic illness known to cause hypoglycemia may be the source .
	manualset3
92052	2	399315	13	NULL	NULL	0	NULL	chronic illness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If these factors are absent , another chronic illness known to cause hypoglycemia may be the source .
	manualset3
92053	3	399315	13	NULL	NULL	0	NULL	hypoglycemia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If these factors are absent , another chronic illness known to cause hypoglycemia may be the source .
	manualset3
98572	4	399315	13	NULL	NULL	0	NULL	 source	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If these factors are absent , another chronic illness known to cause hypoglycemia may be the source .
	manualset3
92054	1	399316	13	NULL	NULL	0	NULL	washin-washout effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	If this , so-called , washin-washout effect is substantial it may interfere with the diagnosis , as a major part of breath HCN may originate from the respiratory tract , due to recent exposure , and not from systemic exposure .
	manualset3
92055	2	399316	13	NULL	NULL	0	NULL	 diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	If this , so-called , washin-washout effect is substantial it may interfere with the diagnosis , as a major part of breath HCN may originate from the respiratory tract , due to recent exposure , and not from systemic exposure .
	manualset3
92056	3	399316	13	NULL	NULL	0	NULL	major part of breath HCN 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	If this , so-called , washin-washout effect is substantial it may interfere with the diagnosis , as a major part of breath HCN may originate from the respiratory tract , due to recent exposure , and not from systemic exposure .
	manualset3
92057	4	399316	13	NULL	NULL	0	NULL	respiratory tract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	If this , so-called , washin-washout effect is substantial it may interfere with the diagnosis , as a major part of breath HCN may originate from the respiratory tract , due to recent exposure , and not from systemic exposure .
	manualset3
92058	5	399316	13	NULL	NULL	NULL	NULL	recent exposure	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	If this , so-called , washin-washout effect is substantial it may interfere with the diagnosis , as a major part of breath HCN may originate from the respiratory tract , due to recent exposure , and not from systemic exposure .
	manualset3
92059	6	399316	13	NULL	NULL	0	NULL	systemic exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	If this , so-called , washin-washout effect is substantial it may interfere with the diagnosis , as a major part of breath HCN may originate from the respiratory tract , due to recent exposure , and not from systemic exposure .
	manualset3
92060	1	399317	13	NULL	NULL	0	NULL	prophylactic infusion therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	If this can be achieved , we may be able to look forward to prophylactic infusion therapy for patients with severe FVIII deficiency and eliminate the significant complications that continue to occur even with prompt treatment of hemorrhage and thrombosis .
	manualset3
92061	2	399317	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	If this can be achieved , we may be able to look forward to prophylactic infusion therapy for patients with severe FVIII deficiency and eliminate the significant complications that continue to occur even with prompt treatment of hemorrhage and thrombosis .
	manualset3
92062	3	399317	13	NULL	NULL	0	NULL	severe FVIII deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If this can be achieved , we may be able to look forward to prophylactic infusion therapy for patients with severe FVIII deficiency and eliminate the significant complications that continue to occur even with prompt treatment of hemorrhage and thrombosis .
	manualset3
92063	4	399317	13	NULL	NULL	0	NULL	significant complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If this can be achieved , we may be able to look forward to prophylactic infusion therapy for patients with severe FVIII deficiency and eliminate the significant complications that continue to occur even with prompt treatment of hemorrhage and thrombosis .
	manualset3
92064	5	399317	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	If this can be achieved , we may be able to look forward to prophylactic infusion therapy for patients with severe FVIII deficiency and eliminate the significant complications that continue to occur even with prompt treatment of hemorrhage and thrombosis .
	manualset3
92065	6	399317	13	NULL	NULL	0	NULL	hemorrhage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If this can be achieved , we may be able to look forward to prophylactic infusion therapy for patients with severe FVIII deficiency and eliminate the significant complications that continue to occur even with prompt treatment of hemorrhage and thrombosis .
	manualset3
92066	7	399317	13	NULL	NULL	0	NULL	thrombosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If this can be achieved , we may be able to look forward to prophylactic infusion therapy for patients with severe FVIII deficiency and eliminate the significant complications that continue to occur even with prompt treatment of hemorrhage and thrombosis .
	manualset3
92067	1	399318	13	NULL	NULL	0	NULL	amidation reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	If true , this would seem to imply that the amidation reaction of the Glut-tRNA ( Gln ) complex was the evolutionary precursor of the direct tRNA ( Gln ) aminoacylation pathway .
	manualset3
92068	2	399318	13	NULL	NULL	0	NULL	Glut-tRNA ( Gln ) complex	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	If true , this would seem to imply that the amidation reaction of the Glut-tRNA ( Gln ) complex was the evolutionary precursor of the direct tRNA ( Gln ) aminoacylation pathway .
	manualset3
92069	3	399318	13	NULL	NULL	0	NULL	evolutionary precursor	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	If true , this would seem to imply that the amidation reaction of the Glut-tRNA ( Gln ) complex was the evolutionary precursor of the direct tRNA ( Gln ) aminoacylation pathway .
	manualset3
92070	4	399318	13	NULL	NULL	0	NULL	direct tRNA ( Gln ) aminoacylation pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	If true , this would seem to imply that the amidation reaction of the Glut-tRNA ( Gln ) complex was the evolutionary precursor of the direct tRNA ( Gln ) aminoacylation pathway .
	manualset3
92071	1	399319	13	NULL	NULL	0	NULL	IgE cross reactivity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IgE cross reactivity between reindeer and bovine milk beta-lactoglobulins in cow 's milk allergic patients .
	manualset3
92072	2	399319	13	NULL	NULL	0	NULL	reindeer milk beta-lactoglobulins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IgE cross reactivity between reindeer and bovine milk beta-lactoglobulins in cow 's milk allergic patients .
	manualset3
92073	3	399319	13	NULL	NULL	0	NULL	bovine milk beta-lactoglobulins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IgE cross reactivity between reindeer and bovine milk beta-lactoglobulins in cow 's milk allergic patients .
	manualset3
92074	4	399319	13	NULL	NULL	0	NULL	cow 's milk allergic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	IgE cross reactivity between reindeer and bovine milk beta-lactoglobulins in cow 's milk allergic patients .
	manualset3
92075	1	399320	13	NULL	NULL	0	NULL	IgG4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IgG4 bound to SG components were found in the sera of the common reaction group at the levels of 24 and 48 kD , but , in one severe case , no bands were observed , although the total IgG was very high .
	manualset3
92076	2	399320	13	NULL	NULL	0	NULL	SG components	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	IgG4 bound to SG components were found in the sera of the common reaction group at the levels of 24 and 48 kD , but , in one severe case , no bands were observed , although the total IgG was very high .
	manualset3
92077	3	399320	13	NULL	NULL	0	NULL	sera	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	IgG4 bound to SG components were found in the sera of the common reaction group at the levels of 24 and 48 kD , but , in one severe case , no bands were observed , although the total IgG was very high .
	manualset3
92078	4	399320	13	NULL	NULL	0	NULL	common reaction group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	IgG4 bound to SG components were found in the sera of the common reaction group at the levels of 24 and 48 kD , but , in one severe case , no bands were observed , although the total IgG was very high .
	manualset3
92079	5	399320	13	NULL	NULL	0	NULL	levels of 24 and 48 kD	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	IgG4 bound to SG components were found in the sera of the common reaction group at the levels of 24 and 48 kD , but , in one severe case , no bands were observed , although the total IgG was very high .
	manualset3
92080	6	399320	13	NULL	NULL	0	NULL	one severe case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	IgG4 bound to SG components were found in the sera of the common reaction group at the levels of 24 and 48 kD , but , in one severe case , no bands were observed , although the total IgG was very high .
	manualset3
92081	7	399320	13	NULL	NULL	0	NULL	total IgG was very high 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	IgG4 bound to SG components were found in the sera of the common reaction group at the levels of 24 and 48 kD , but , in one severe case , no bands were observed , although the total IgG was very high .
	manualset3
92082	1	399321	13	NULL	NULL	NULL	NULL	IgM concentrations	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	IgM concentrations were significantly ( P = .002 ) higher in the affected dogs ( median 1.95 mg/mL ) than in the control dogs ( median 1.12 mg/mL ) .
	manualset3
92083	2	399321	13	NULL	NULL	0	NULL	 ( P = .002 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	IgM concentrations were significantly ( P = .002 ) higher in the affected dogs ( median 1.95 mg/mL ) than in the control dogs ( median 1.12 mg/mL ) .
	manualset3
92084	3	399321	13	NULL	NULL	0	NULL	dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	IgM concentrations were significantly ( P = .002 ) higher in the affected dogs ( median 1.95 mg/mL ) than in the control dogs ( median 1.12 mg/mL ) .
	manualset3
92085	4	399321	13	NULL	NULL	0	NULL	median 1.95 mg/mL 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	IgM concentrations were significantly ( P = .002 ) higher in the affected dogs ( median 1.95 mg/mL ) than in the control dogs ( median 1.12 mg/mL ) .
	manualset3
92086	5	399321	13	NULL	NULL	0	NULL	control dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	IgM concentrations were significantly ( P = .002 ) higher in the affected dogs ( median 1.95 mg/mL ) than in the control dogs ( median 1.12 mg/mL ) .
	manualset3
92087	6	399321	13	NULL	NULL	0	NULL	median 1.12 mg/mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	IgM concentrations were significantly ( P = .002 ) higher in the affected dogs ( median 1.95 mg/mL ) than in the control dogs ( median 1.12 mg/mL ) .
	manualset3
92088	1	399322	13	NULL	NULL	0	NULL	diffusion-related NaCl effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ignoring the presumably diffusion-related NaCl effect on carbon isotope ratios results in an overestimation of nocturnal CO ( 2 ) gain in comparison to an isotope versus nocturnal CO ( 2 ) gain calibration established previously for C ( 3 ) and CAM species grown under well-watered conditions .
	manualset3
92089	2	399322	13	NULL	NULL	0	NULL	carbon isotope ratios	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ignoring the presumably diffusion-related NaCl effect on carbon isotope ratios results in an overestimation of nocturnal CO ( 2 ) gain in comparison to an isotope versus nocturnal CO ( 2 ) gain calibration established previously for C ( 3 ) and CAM species grown under well-watered conditions .
	manualset3
92090	3	399322	13	NULL	NULL	0	NULL	overestimation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ignoring the presumably diffusion-related NaCl effect on carbon isotope ratios results in an overestimation of nocturnal CO ( 2 ) gain in comparison to an isotope versus nocturnal CO ( 2 ) gain calibration established previously for C ( 3 ) and CAM species grown under well-watered conditions .
	manualset3
92091	4	399322	13	NULL	NULL	0	NULL	nocturnal CO ( 2 ) gain	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ignoring the presumably diffusion-related NaCl effect on carbon isotope ratios results in an overestimation of nocturnal CO ( 2 ) gain in comparison to an isotope versus nocturnal CO ( 2 ) gain calibration established previously for C ( 3 ) and CAM species grown under well-watered conditions .
	manualset3
92092	5	399322	13	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Ignoring the presumably diffusion-related NaCl effect on carbon isotope ratios results in an overestimation of nocturnal CO ( 2 ) gain in comparison to an isotope versus nocturnal CO ( 2 ) gain calibration established previously for C ( 3 ) and CAM species grown under well-watered conditions .
	manualset3
92093	6	399322	13	NULL	NULL	0	NULL	isotope versus nocturnal CO ( 2 ) gain calibration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ignoring the presumably diffusion-related NaCl effect on carbon isotope ratios results in an overestimation of nocturnal CO ( 2 ) gain in comparison to an isotope versus nocturnal CO ( 2 ) gain calibration established previously for C ( 3 ) and CAM species grown under well-watered conditions .
	manualset3
92094	7	399322	13	NULL	NULL	0	NULL	C ( 3 ) species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ignoring the presumably diffusion-related NaCl effect on carbon isotope ratios results in an overestimation of nocturnal CO ( 2 ) gain in comparison to an isotope versus nocturnal CO ( 2 ) gain calibration established previously for C ( 3 ) and CAM species grown under well-watered conditions .
	manualset3
92095	8	399322	13	NULL	NULL	0	NULL	CAM species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ignoring the presumably diffusion-related NaCl effect on carbon isotope ratios results in an overestimation of nocturnal CO ( 2 ) gain in comparison to an isotope versus nocturnal CO ( 2 ) gain calibration established previously for C ( 3 ) and CAM species grown under well-watered conditions .
	manualset3
92096	9	399322	13	NULL	NULL	0	NULL	conditions	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Ignoring the presumably diffusion-related NaCl effect on carbon isotope ratios results in an overestimation of nocturnal CO ( 2 ) gain in comparison to an isotope versus nocturnal CO ( 2 ) gain calibration established previously for C ( 3 ) and CAM species grown under well-watered conditions .
	manualset3
92097	1	399323	13	NULL	NULL	NULL	NULL	value of sex chromatin	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The value of sex chromatin in the hormone therapy of breast tumors ) .
	manualset3
92098	2	399323	13	NULL	NULL	0	NULL	 hormone therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( The value of sex chromatin in the hormone therapy of breast tumors ) .
	manualset3
92099	3	399323	13	NULL	NULL	0	NULL	breast tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( The value of sex chromatin in the hormone therapy of breast tumors ) .
	manualset3
92100	1	399324	13	NULL	NULL	0	NULL	Image stacks	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Image stacks ( 5 benign , 7 malignant tumors ) were analyzed by established software ( principal component analysis PCA , hyperspectral classification , spectral profiles ) .
	manualset3
92101	2	399324	13	NULL	NULL	0	NULL	5	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Image stacks ( 5 benign , 7 malignant tumors ) were analyzed by established software ( principal component analysis PCA , hyperspectral classification , spectral profiles ) .
	manualset3
92102	3	399324	13	NULL	NULL	0	NULL	benign tumors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Image stacks ( 5 benign , 7 malignant tumors ) were analyzed by established software ( principal component analysis PCA , hyperspectral classification , spectral profiles ) .
	manualset3
92103	4	399324	13	NULL	NULL	0	NULL	7	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Image stacks ( 5 benign , 7 malignant tumors ) were analyzed by established software ( principal component analysis PCA , hyperspectral classification , spectral profiles ) .
	manualset3
92104	5	399324	13	NULL	NULL	0	NULL	 malignant tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Image stacks ( 5 benign , 7 malignant tumors ) were analyzed by established software ( principal component analysis PCA , hyperspectral classification , spectral profiles ) .
	manualset3
92105	6	399324	13	NULL	NULL	0	NULL	software	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Image stacks ( 5 benign , 7 malignant tumors ) were analyzed by established software ( principal component analysis PCA , hyperspectral classification , spectral profiles ) .
	manualset3
92106	7	399324	13	NULL	NULL	0	NULL	principal component analysis PCA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Image stacks ( 5 benign , 7 malignant tumors ) were analyzed by established software ( principal component analysis PCA , hyperspectral classification , spectral profiles ) .
	manualset3
92107	8	399324	13	NULL	NULL	0	NULL	 hyperspectral classification	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Image stacks ( 5 benign , 7 malignant tumors ) were analyzed by established software ( principal component analysis PCA , hyperspectral classification , spectral profiles ) .
	manualset3
92108	9	399324	13	NULL	NULL	0	NULL	spectral profiles	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Image stacks ( 5 benign , 7 malignant tumors ) were analyzed by established software ( principal component analysis PCA , hyperspectral classification , spectral profiles ) .
	manualset3
92109	1	399325	13	NULL	NULL	0	NULL	Images of tooth slices	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Images of tooth slices were also visually examined under magnification and dye penetration along the tooth/restoration interface was scored .
	manualset3
92110	2	399325	13	NULL	NULL	0	NULL	magnification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Images of tooth slices were also visually examined under magnification and dye penetration along the tooth/restoration interface was scored .
	manualset3
92111	3	399325	13	NULL	NULL	0	NULL	dye penetration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Images of tooth slices were also visually examined under magnification and dye penetration along the tooth/restoration interface was scored .
	manualset3
92112	4	399325	13	NULL	NULL	0	NULL	tooth/restoration interface	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Images of tooth slices were also visually examined under magnification and dye penetration along the tooth/restoration interface was scored .
	manualset3
92113	1	399326	13	NULL	NULL	0	NULL	Images	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Images were taken using single breath-hold and ECG triggering .
	manualset3
92114	2	399326	13	NULL	NULL	0	NULL	single breath-hold 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Images were taken using single breath-hold and ECG triggering .
	manualset3
92115	3	399326	13	NULL	NULL	0	NULL	 ECG triggering	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Images were taken using single breath-hold and ECG triggering .
	manualset3
92116	1	399327	13	NULL	NULL	0	NULL	topic	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Imaging is the topic of 1998 with advances in the areas of ultrasound .
	manualset3
92117	2	399327	13	NULL	NULL	0	NULL	1998	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Imaging is the topic of 1998 with advances in the areas of ultrasound .
	manualset3
92118	3	399327	13	NULL	NULL	0	NULL	areas of ultrasound	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Imaging is the topic of 1998 with advances in the areas of ultrasound .
	manualset3
98573	4	399327	13	NULL	NULL	0	NULL	Imaging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Imaging is the topic of 1998 with advances in the areas of ultrasound .
	manualset3
92119	1	399328	13	NULL	NULL	0	NULL	 important role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Imaging plays an important role in LDLT programs by providing robust evaluation of potential donors to ensure that only anatomically suitable donors with no significant co-existing pathology are selected and that crucial information that allows detailed preoperative planning is available .
	manualset3
92120	2	399328	13	NULL	NULL	0	NULL	LDLT programs	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Imaging plays an important role in LDLT programs by providing robust evaluation of potential donors to ensure that only anatomically suitable donors with no significant co-existing pathology are selected and that crucial information that allows detailed preoperative planning is available .
	manualset3
92121	3	399328	13	NULL	NULL	0	NULL	 robust evaluation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Imaging plays an important role in LDLT programs by providing robust evaluation of potential donors to ensure that only anatomically suitable donors with no significant co-existing pathology are selected and that crucial information that allows detailed preoperative planning is available .
	manualset3
92122	4	399328	13	NULL	NULL	0	NULL	potential donors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Imaging plays an important role in LDLT programs by providing robust evaluation of potential donors to ensure that only anatomically suitable donors with no significant co-existing pathology are selected and that crucial information that allows detailed preoperative planning is available .
	manualset3
92123	5	399328	13	NULL	NULL	NULL	NULL	suitable donors	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Imaging plays an important role in LDLT programs by providing robust evaluation of potential donors to ensure that only anatomically suitable donors with no significant co-existing pathology are selected and that crucial information that allows detailed preoperative planning is available .
	manualset3
92124	6	399328	13	NULL	NULL	0	NULL	pathology 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Imaging plays an important role in LDLT programs by providing robust evaluation of potential donors to ensure that only anatomically suitable donors with no significant co-existing pathology are selected and that crucial information that allows detailed preoperative planning is available .
	manualset3
92125	7	399328	13	NULL	NULL	0	NULL	crucial information	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Imaging plays an important role in LDLT programs by providing robust evaluation of potential donors to ensure that only anatomically suitable donors with no significant co-existing pathology are selected and that crucial information that allows detailed preoperative planning is available .
	manualset3
98574	8	399328	13	NULL	NULL	0	NULL	Imaging 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Imaging plays an important role in LDLT programs by providing robust evaluation of potential donors to ensure that only anatomically suitable donors with no significant co-existing pathology are selected and that crucial information that allows detailed preoperative planning is available .
	manualset3
92126	1	399329	13	NULL	NULL	0	NULL	hematopoietic stem cell transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Imaging in hematopoietic stem cell transplantation .
	manualset3
98575	2	399329	13	NULL	NULL	0	NULL	Imaging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Imaging in hematopoietic stem cell transplantation .
	manualset3
92127	2	399330	13	NULL	NULL	NULL	NULL	acute neurological conditions 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Imaging of acute neurological conditions in pregnancy and the puerperium .
	manualset3
92128	3	399330	13	NULL	NULL	NULL	NULL	pregnancy	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Imaging of acute neurological conditions in pregnancy and the puerperium .
	manualset3
92129	4	399330	13	NULL	NULL	NULL	NULL	puerperium	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Imaging of acute neurological conditions in pregnancy and the puerperium .
	manualset3
94202	1	399330	13	NULL	NULL	NULL	NULL	Imaging	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Imaging of acute neurological conditions in pregnancy and the puerperium .
	manualset3
92397	2	399331	13	NULL	NULL	NULL	NULL	primary penile cancer	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Imaging of primary penile cancer and metastatic lymphadenopathy can help optimize planning of both primary tumor resection and treatment for lymph node metastases .
	manualset3
92406	3	399331	13	NULL	NULL	NULL	NULL	metastatic lymphadenopathy	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Imaging of primary penile cancer and metastatic lymphadenopathy can help optimize planning of both primary tumor resection and treatment for lymph node metastases .
	manualset3
92410	5	399331	13	NULL	NULL	NULL	NULL	primary tumor resection	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Imaging of primary penile cancer and metastatic lymphadenopathy can help optimize planning of both primary tumor resection and treatment for lymph node metastases .
	manualset3
92411	6	399331	13	NULL	NULL	NULL	NULL	treatment 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Imaging of primary penile cancer and metastatic lymphadenopathy can help optimize planning of both primary tumor resection and treatment for lymph node metastases .
	manualset3
92412	7	399331	13	NULL	NULL	NULL	NULL	lymph node metastases 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Imaging of primary penile cancer and metastatic lymphadenopathy can help optimize planning of both primary tumor resection and treatment for lymph node metastases .
	manualset3
94203	1	399331	13	NULL	NULL	0	NULL	Imaging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Imaging of primary penile cancer and metastatic lymphadenopathy can help optimize planning of both primary tumor resection and treatment for lymph node metastases .
	manualset3
94204	4	399331	13	NULL	NULL	0	NULL	optimize planning	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Imaging of primary penile cancer and metastatic lymphadenopathy can help optimize planning of both primary tumor resection and treatment for lymph node metastases .
	manualset3
92414	4	399332	13	NULL	NULL	NULL	NULL	protease functions	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Imaging of protease functions -- current guide to spotting cysteine cathepsins in classical and novel scenes of action in mammalian epithelial cells and tissues .
	manualset3
92419	2	399332	13	NULL	NULL	0	NULL	cysteine cathepsins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Imaging of protease functions -- current guide to spotting cysteine cathepsins in classical and novel scenes of action in mammalian epithelial cells and tissues .
	manualset3
92421	5	399332	13	NULL	NULL	NULL	NULL	classical scenes of action	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Imaging of protease functions -- current guide to spotting cysteine cathepsins in classical and novel scenes of action in mammalian epithelial cells and tissues .
	manualset3
92422	6	399332	13	NULL	NULL	NULL	NULL	novel scenes of action	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Imaging of protease functions -- current guide to spotting cysteine cathepsins in classical and novel scenes of action in mammalian epithelial cells and tissues .
	manualset3
92423	7	399332	13	NULL	NULL	NULL	NULL	mammalian epithelial cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Imaging of protease functions -- current guide to spotting cysteine cathepsins in classical and novel scenes of action in mammalian epithelial cells and tissues .
	manualset3
92424	8	399332	13	NULL	NULL	NULL	NULL	mammalian epithelial tissues	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Imaging of protease functions -- current guide to spotting cysteine cathepsins in classical and novel scenes of action in mammalian epithelial cells and tissues .
	manualset3
94205	1	399332	13	NULL	NULL	0	NULL	Imaging	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Imaging of protease functions -- current guide to spotting cysteine cathepsins in classical and novel scenes of action in mammalian epithelial cells and tissues .
	manualset3
94206	3	399332	13	NULL	NULL	NULL	NULL	guide	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Imaging of protease functions -- current guide to spotting cysteine cathepsins in classical and novel scenes of action in mammalian epithelial cells and tissues .
	manualset3
92425	1	399333	13	NULL	NULL	NULL	NULL	Imaging of the vascular system	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Imaging of the vascular system revealed vessels down to the caliber of capillaries , and the digital three-dimensional data obtained from the scans allowed for virtual cutting , amplification , and scaling without destroying the sample .
	manualset3
92428	2	399333	13	NULL	NULL	0	NULL	vessels 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Imaging of the vascular system revealed vessels down to the caliber of capillaries , and the digital three-dimensional data obtained from the scans allowed for virtual cutting , amplification , and scaling without destroying the sample .
	manualset3
92430	3	399333	13	NULL	NULL	0	NULL	caliber of capillaries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Imaging of the vascular system revealed vessels down to the caliber of capillaries , and the digital three-dimensional data obtained from the scans allowed for virtual cutting , amplification , and scaling without destroying the sample .
	manualset3
92497	4	399333	13	NULL	NULL	0	NULL	digital three-dimensional data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Imaging of the vascular system revealed vessels down to the caliber of capillaries , and the digital three-dimensional data obtained from the scans allowed for virtual cutting , amplification , and scaling without destroying the sample .
	manualset3
92502	5	399333	13	NULL	NULL	0	NULL	scans 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Imaging of the vascular system revealed vessels down to the caliber of capillaries , and the digital three-dimensional data obtained from the scans allowed for virtual cutting , amplification , and scaling without destroying the sample .
	manualset3
92508	7	399333	13	NULL	NULL	NULL	NULL	 amplification 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Imaging of the vascular system revealed vessels down to the caliber of capillaries , and the digital three-dimensional data obtained from the scans allowed for virtual cutting , amplification , and scaling without destroying the sample .
	manualset3
92509	8	399333	13	NULL	NULL	NULL	NULL	sample	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Imaging of the vascular system revealed vessels down to the caliber of capillaries , and the digital three-dimensional data obtained from the scans allowed for virtual cutting , amplification , and scaling without destroying the sample .
	manualset3
94208	6	399333	13	NULL	NULL	0	NULL	 virtual cutting	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Imaging of the vascular system revealed vessels down to the caliber of capillaries , and the digital three-dimensional data obtained from the scans allowed for virtual cutting , amplification , and scaling without destroying the sample .
	manualset3
92512	1	399334	13	NULL	NULL	0	NULL	historical development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Then and now ; the historical development of the theory of pernicious anemia Biermer ) .
	manualset3
92516	2	399334	13	NULL	NULL	0	NULL	theory	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Then and now ; the historical development of the theory of pernicious anemia Biermer ) .
	manualset3
92517	3	399334	13	NULL	NULL	0	NULL	pernicious anemia Biermer	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Then and now ; the historical development of the theory of pernicious anemia Biermer ) .
	manualset3
96842	4	399334	13	NULL	NULL	0	NULL	Then	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	( Then and now ; the historical development of the theory of pernicious anemia Biermer ) .
	manualset3
96843	5	399334	13	NULL	NULL	0	NULL	now	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	( Then and now ; the historical development of the theory of pernicious anemia Biermer ) .
	manualset3
92518	1	399335	13	NULL	NULL	0	NULL	Iminoazophenol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Iminoazophenol appended calix ( 4 ) arene/thiacalix ( 4 ) arene derivatives 1 and 2 of cone and 3 of 1 , 3-alternate conformation have been synthesized and examined for their chromogenic anion recognition abilities towards different anions like fluoride , chloride , bromide , iodide , acetate , dihydrogenphosphate , nitrate and hydrogensulphate by UV-vis spectroscopy .
	manualset3
92519	2	399335	13	NULL	NULL	NULL	NULL	 calix ( 4 ) arene/thiacalix ( 4 ) arene derivatives 1	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Iminoazophenol appended calix ( 4 ) arene/thiacalix ( 4 ) arene derivatives 1 and 2 of cone and 3 of 1 , 3-alternate conformation have been synthesized and examined for their chromogenic anion recognition abilities towards different anions like fluoride , chloride , bromide , iodide , acetate , dihydrogenphosphate , nitrate and hydrogensulphate by UV-vis spectroscopy .
	manualset3
92520	3	399335	13	NULL	NULL	NULL	NULL	 calix ( 4 ) arene/thiacalix ( 4 ) arene derivatives 2	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Iminoazophenol appended calix ( 4 ) arene/thiacalix ( 4 ) arene derivatives 1 and 2 of cone and 3 of 1 , 3-alternate conformation have been synthesized and examined for their chromogenic anion recognition abilities towards different anions like fluoride , chloride , bromide , iodide , acetate , dihydrogenphosphate , nitrate and hydrogensulphate by UV-vis spectroscopy .
	manualset3
92522	5	399335	13	NULL	NULL	0	NULL	 3 of 1 , 3-alternate conformation	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Iminoazophenol appended calix ( 4 ) arene/thiacalix ( 4 ) arene derivatives 1 and 2 of cone and 3 of 1 , 3-alternate conformation have been synthesized and examined for their chromogenic anion recognition abilities towards different anions like fluoride , chloride , bromide , iodide , acetate , dihydrogenphosphate , nitrate and hydrogensulphate by UV-vis spectroscopy .
	manualset3
92523	6	399335	13	NULL	NULL	0	NULL	chromogenic anion 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Iminoazophenol appended calix ( 4 ) arene/thiacalix ( 4 ) arene derivatives 1 and 2 of cone and 3 of 1 , 3-alternate conformation have been synthesized and examined for their chromogenic anion recognition abilities towards different anions like fluoride , chloride , bromide , iodide , acetate , dihydrogenphosphate , nitrate and hydrogensulphate by UV-vis spectroscopy .
	manualset3
92524	7	399335	13	NULL	NULL	0	NULL	recognition abilities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Iminoazophenol appended calix ( 4 ) arene/thiacalix ( 4 ) arene derivatives 1 and 2 of cone and 3 of 1 , 3-alternate conformation have been synthesized and examined for their chromogenic anion recognition abilities towards different anions like fluoride , chloride , bromide , iodide , acetate , dihydrogenphosphate , nitrate and hydrogensulphate by UV-vis spectroscopy .
	manualset3
92525	8	399335	13	NULL	NULL	0	NULL	anions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Iminoazophenol appended calix ( 4 ) arene/thiacalix ( 4 ) arene derivatives 1 and 2 of cone and 3 of 1 , 3-alternate conformation have been synthesized and examined for their chromogenic anion recognition abilities towards different anions like fluoride , chloride , bromide , iodide , acetate , dihydrogenphosphate , nitrate and hydrogensulphate by UV-vis spectroscopy .
	manualset3
92526	9	399335	13	NULL	NULL	0	NULL	fluoride	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Iminoazophenol appended calix ( 4 ) arene/thiacalix ( 4 ) arene derivatives 1 and 2 of cone and 3 of 1 , 3-alternate conformation have been synthesized and examined for their chromogenic anion recognition abilities towards different anions like fluoride , chloride , bromide , iodide , acetate , dihydrogenphosphate , nitrate and hydrogensulphate by UV-vis spectroscopy .
	manualset3
92527	10	399335	13	NULL	NULL	0	NULL	 chloride	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Iminoazophenol appended calix ( 4 ) arene/thiacalix ( 4 ) arene derivatives 1 and 2 of cone and 3 of 1 , 3-alternate conformation have been synthesized and examined for their chromogenic anion recognition abilities towards different anions like fluoride , chloride , bromide , iodide , acetate , dihydrogenphosphate , nitrate and hydrogensulphate by UV-vis spectroscopy .
	manualset3
92528	11	399335	13	NULL	NULL	0	NULL	bromide	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Iminoazophenol appended calix ( 4 ) arene/thiacalix ( 4 ) arene derivatives 1 and 2 of cone and 3 of 1 , 3-alternate conformation have been synthesized and examined for their chromogenic anion recognition abilities towards different anions like fluoride , chloride , bromide , iodide , acetate , dihydrogenphosphate , nitrate and hydrogensulphate by UV-vis spectroscopy .
	manualset3
92529	12	399335	13	NULL	NULL	0	NULL	 iodide	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Iminoazophenol appended calix ( 4 ) arene/thiacalix ( 4 ) arene derivatives 1 and 2 of cone and 3 of 1 , 3-alternate conformation have been synthesized and examined for their chromogenic anion recognition abilities towards different anions like fluoride , chloride , bromide , iodide , acetate , dihydrogenphosphate , nitrate and hydrogensulphate by UV-vis spectroscopy .
	manualset3
92530	13	399335	13	NULL	NULL	0	NULL	acetate	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Iminoazophenol appended calix ( 4 ) arene/thiacalix ( 4 ) arene derivatives 1 and 2 of cone and 3 of 1 , 3-alternate conformation have been synthesized and examined for their chromogenic anion recognition abilities towards different anions like fluoride , chloride , bromide , iodide , acetate , dihydrogenphosphate , nitrate and hydrogensulphate by UV-vis spectroscopy .
	manualset3
92531	14	399335	13	NULL	NULL	0	NULL	dihydrogenphosphate 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Iminoazophenol appended calix ( 4 ) arene/thiacalix ( 4 ) arene derivatives 1 and 2 of cone and 3 of 1 , 3-alternate conformation have been synthesized and examined for their chromogenic anion recognition abilities towards different anions like fluoride , chloride , bromide , iodide , acetate , dihydrogenphosphate , nitrate and hydrogensulphate by UV-vis spectroscopy .
	manualset3
92532	15	399335	13	NULL	NULL	0	NULL	nitrate	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Iminoazophenol appended calix ( 4 ) arene/thiacalix ( 4 ) arene derivatives 1 and 2 of cone and 3 of 1 , 3-alternate conformation have been synthesized and examined for their chromogenic anion recognition abilities towards different anions like fluoride , chloride , bromide , iodide , acetate , dihydrogenphosphate , nitrate and hydrogensulphate by UV-vis spectroscopy .
	manualset3
92533	16	399335	13	NULL	NULL	0	NULL	hydrogensulphate 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Iminoazophenol appended calix ( 4 ) arene/thiacalix ( 4 ) arene derivatives 1 and 2 of cone and 3 of 1 , 3-alternate conformation have been synthesized and examined for their chromogenic anion recognition abilities towards different anions like fluoride , chloride , bromide , iodide , acetate , dihydrogenphosphate , nitrate and hydrogensulphate by UV-vis spectroscopy .
	manualset3
92534	17	399335	13	NULL	NULL	0	NULL	UV-vis spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Iminoazophenol appended calix ( 4 ) arene/thiacalix ( 4 ) arene derivatives 1 and 2 of cone and 3 of 1 , 3-alternate conformation have been synthesized and examined for their chromogenic anion recognition abilities towards different anions like fluoride , chloride , bromide , iodide , acetate , dihydrogenphosphate , nitrate and hydrogensulphate by UV-vis spectroscopy .
	manualset3
92577	1	399336	13	NULL	NULL	NULL	NULL	Immediate effects	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immediate and long-term effects of addition of exercise to a 16-week very low calorie diet on low-grade inflammation in obese , insulin-dependent type 2 diabetic patients .
	manualset3
92578	2	399336	13	NULL	NULL	NULL	NULL	 long-term effects 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immediate and long-term effects of addition of exercise to a 16-week very low calorie diet on low-grade inflammation in obese , insulin-dependent type 2 diabetic patients .
	manualset3
92579	3	399336	13	NULL	NULL	0	NULL	addition of exercise 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Immediate and long-term effects of addition of exercise to a 16-week very low calorie diet on low-grade inflammation in obese , insulin-dependent type 2 diabetic patients .
	manualset3
92580	4	399336	13	NULL	NULL	0	NULL	16-week	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Immediate and long-term effects of addition of exercise to a 16-week very low calorie diet on low-grade inflammation in obese , insulin-dependent type 2 diabetic patients .
	manualset3
92581	5	399336	13	NULL	NULL	0	NULL	low calorie diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Immediate and long-term effects of addition of exercise to a 16-week very low calorie diet on low-grade inflammation in obese , insulin-dependent type 2 diabetic patients .
	manualset3
92582	6	399336	13	NULL	NULL	0	NULL	low-grade inflammation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immediate and long-term effects of addition of exercise to a 16-week very low calorie diet on low-grade inflammation in obese , insulin-dependent type 2 diabetic patients .
	manualset3
92583	7	399336	13	NULL	NULL	0	NULL	obese patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Immediate and long-term effects of addition of exercise to a 16-week very low calorie diet on low-grade inflammation in obese , insulin-dependent type 2 diabetic patients .
	manualset3
92584	8	399336	13	NULL	NULL	0	NULL	insulin-dependent type 2 diabetic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Immediate and long-term effects of addition of exercise to a 16-week very low calorie diet on low-grade inflammation in obese , insulin-dependent type 2 diabetic patients .
	manualset3
92585	2	399337	13	NULL	NULL	NULL	NULL	larger initial specimens	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immediate re-sampling , or larger initial specimens would have salvaged the procedure in most instances of failure .
	manualset3
92586	2	399337	13	NULL	NULL	0	NULL	procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Immediate re-sampling , or larger initial specimens would have salvaged the procedure in most instances of failure .
	manualset3
92587	3	399337	13	NULL	NULL	0	NULL	instances of failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immediate re-sampling , or larger initial specimens would have salvaged the procedure in most instances of failure .
	manualset3
94209	1	399337	13	NULL	NULL	0	NULL	Immediate re-sampling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immediate re-sampling , or larger initial specimens would have salvaged the procedure in most instances of failure .
	manualset3
92588	1	399338	13	NULL	NULL	0	NULL	Immobilization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Immobilization of protamine to the inner lumen of cellulose hollow fibers has been shown useful in preventing both heparin - and protamine-induced complications during an extracorporeal blood circulation procedure .
	manualset3
92589	2	399338	13	NULL	NULL	0	NULL	protamine	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immobilization of protamine to the inner lumen of cellulose hollow fibers has been shown useful in preventing both heparin - and protamine-induced complications during an extracorporeal blood circulation procedure .
	manualset3
92590	3	399338	13	NULL	NULL	NULL	NULL	inner lumen of cellulose hollow fibers	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immobilization of protamine to the inner lumen of cellulose hollow fibers has been shown useful in preventing both heparin - and protamine-induced complications during an extracorporeal blood circulation procedure .
	manualset3
92591	4	399338	13	NULL	NULL	0	NULL	heparin-induced complications 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immobilization of protamine to the inner lumen of cellulose hollow fibers has been shown useful in preventing both heparin - and protamine-induced complications during an extracorporeal blood circulation procedure .
	manualset3
92592	5	399338	13	NULL	NULL	0	NULL	protamine-induced complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immobilization of protamine to the inner lumen of cellulose hollow fibers has been shown useful in preventing both heparin - and protamine-induced complications during an extracorporeal blood circulation procedure .
	manualset3
92593	6	399338	13	NULL	NULL	0	NULL	 extracorporeal blood circulation procedure 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Immobilization of protamine to the inner lumen of cellulose hollow fibers has been shown useful in preventing both heparin - and protamine-induced complications during an extracorporeal blood circulation procedure .
	manualset3
92594	1	399339	13	NULL	NULL	0	NULL	Immune cytokine inhibition 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Immune cytokine inhibition of beta-adrenergic agonist stimulated cyclic AMP generation in cardiac myocytes .
	manualset3
92595	2	399339	13	NULL	NULL	0	NULL	beta-adrenergic agonist	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Immune cytokine inhibition of beta-adrenergic agonist stimulated cyclic AMP generation in cardiac myocytes .
	manualset3
92596	3	399339	13	NULL	NULL	0	NULL	cyclic AMP generation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Immune cytokine inhibition of beta-adrenergic agonist stimulated cyclic AMP generation in cardiac myocytes .
	manualset3
92597	4	399339	13	NULL	NULL	0	NULL	cardiac myocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Immune cytokine inhibition of beta-adrenergic agonist stimulated cyclic AMP generation in cardiac myocytes .
	manualset3
92598	1	399340	13	NULL	NULL	0	NULL	Therapeutic action	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Therapeutic and prophylactic action of succimer in experimental subacute lead acetate poisoning ) .
	manualset3
92599	2	399340	13	NULL	NULL	0	NULL	prophylactic action 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Therapeutic and prophylactic action of succimer in experimental subacute lead acetate poisoning ) .
	manualset3
92600	3	399340	13	NULL	NULL	0	NULL	succimer	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Therapeutic and prophylactic action of succimer in experimental subacute lead acetate poisoning ) .
	manualset3
92601	4	399340	13	NULL	NULL	NULL	NULL	experimental subacute lead acetate poisoning	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Therapeutic and prophylactic action of succimer in experimental subacute lead acetate poisoning ) .
	manualset3
92602	1	399341	13	NULL	NULL	0	NULL	Immune factors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immune factors such as cellular immunity , autoimmunity , and inflammation may play a pathogenic role in Alzheimer 's disease ( AD ) , a neurodegenerative disorder .
	manualset3
92603	2	399341	13	NULL	NULL	NULL	NULL	cellular immunity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immune factors such as cellular immunity , autoimmunity , and inflammation may play a pathogenic role in Alzheimer 's disease ( AD ) , a neurodegenerative disorder .
	manualset3
92604	3	399341	13	NULL	NULL	0	NULL	autoimmunity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immune factors such as cellular immunity , autoimmunity , and inflammation may play a pathogenic role in Alzheimer 's disease ( AD ) , a neurodegenerative disorder .
	manualset3
92605	4	399341	13	NULL	NULL	0	NULL	inflammation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immune factors such as cellular immunity , autoimmunity , and inflammation may play a pathogenic role in Alzheimer 's disease ( AD ) , a neurodegenerative disorder .
	manualset3
92606	5	399341	13	NULL	NULL	0	NULL	pathogenic role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immune factors such as cellular immunity , autoimmunity , and inflammation may play a pathogenic role in Alzheimer 's disease ( AD ) , a neurodegenerative disorder .
	manualset3
92607	6	399341	13	NULL	NULL	0	NULL	Alzheimer 's disease ( AD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Immune factors such as cellular immunity , autoimmunity , and inflammation may play a pathogenic role in Alzheimer 's disease ( AD ) , a neurodegenerative disorder .
	manualset3
92608	7	399341	13	NULL	NULL	0	NULL	neurodegenerative disorder 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Immune factors such as cellular immunity , autoimmunity , and inflammation may play a pathogenic role in Alzheimer 's disease ( AD ) , a neurodegenerative disorder .
	manualset3
92609	1	399342	13	NULL	NULL	0	NULL	Immune reactivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immune reactivity of the purified hemagglutinin of measles virus .
	manualset3
92610	2	399342	13	NULL	NULL	0	NULL	hemagglutinin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immune reactivity of the purified hemagglutinin of measles virus .
	manualset3
92611	3	399342	13	NULL	NULL	0	NULL	 measles virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Immune reactivity of the purified hemagglutinin of measles virus .
	manualset3
92612	1	399343	13	NULL	NULL	0	NULL	Immunisation coverage	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunisation coverage with 3 doses of oral polio vaccine ( OPV ) was less than 10 % during 1974-80 when immunisation was a clinic based activity .
	manualset3
92613	2	399343	13	NULL	NULL	0	NULL	3 doses of oral polio vaccine ( OPV ) 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunisation coverage with 3 doses of oral polio vaccine ( OPV ) was less than 10 % during 1974-80 when immunisation was a clinic based activity .
	manualset3
92614	3	399343	13	NULL	NULL	0	NULL	less than 10 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunisation coverage with 3 doses of oral polio vaccine ( OPV ) was less than 10 % during 1974-80 when immunisation was a clinic based activity .
	manualset3
92615	4	399343	13	NULL	NULL	0	NULL	1974-80	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunisation coverage with 3 doses of oral polio vaccine ( OPV ) was less than 10 % during 1974-80 when immunisation was a clinic based activity .
	manualset3
92616	5	399343	13	NULL	NULL	0	NULL	 immunisation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunisation coverage with 3 doses of oral polio vaccine ( OPV ) was less than 10 % during 1974-80 when immunisation was a clinic based activity .
	manualset3
92617	6	399343	13	NULL	NULL	0	NULL	 clinic based activity	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunisation coverage with 3 doses of oral polio vaccine ( OPV ) was less than 10 % during 1974-80 when immunisation was a clinic based activity .
	manualset3
92618	1	399344	13	NULL	NULL	0	NULL	Immunization 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunization against a dominant tumor antigen abrogates immunogenicity of the tumor .
	manualset3
92619	2	399344	13	NULL	NULL	0	NULL	dominant tumor antigen	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunization against a dominant tumor antigen abrogates immunogenicity of the tumor .
	manualset3
92620	3	399344	13	NULL	NULL	0	NULL	immunogenicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunization against a dominant tumor antigen abrogates immunogenicity of the tumor .
	manualset3
92621	4	399344	13	NULL	NULL	0	NULL	tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunization against a dominant tumor antigen abrogates immunogenicity of the tumor .
	manualset3
92622	1	399345	13	NULL	NULL	0	NULL	Immunization 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunization of children with asthma against pneumococcal infection with polysaccharide vaccine or combined immunization against pneumococcal infection and influenza reduced rate of asthma exacerbations and led to formation of immunity to vaccine strains of Streptococcus pneumoniae .
	manualset3
92623	2	399345	13	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunization of children with asthma against pneumococcal infection with polysaccharide vaccine or combined immunization against pneumococcal infection and influenza reduced rate of asthma exacerbations and led to formation of immunity to vaccine strains of Streptococcus pneumoniae .
	manualset3
92624	3	399345	13	NULL	NULL	0	NULL	asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunization of children with asthma against pneumococcal infection with polysaccharide vaccine or combined immunization against pneumococcal infection and influenza reduced rate of asthma exacerbations and led to formation of immunity to vaccine strains of Streptococcus pneumoniae .
	manualset3
92625	4	399345	13	NULL	NULL	0	NULL	pneumococcal infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunization of children with asthma against pneumococcal infection with polysaccharide vaccine or combined immunization against pneumococcal infection and influenza reduced rate of asthma exacerbations and led to formation of immunity to vaccine strains of Streptococcus pneumoniae .
	manualset3
92626	5	399345	13	NULL	NULL	0	NULL	polysaccharide vaccine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunization of children with asthma against pneumococcal infection with polysaccharide vaccine or combined immunization against pneumococcal infection and influenza reduced rate of asthma exacerbations and led to formation of immunity to vaccine strains of Streptococcus pneumoniae .
	manualset3
92627	6	399345	13	NULL	NULL	0	NULL	immunization 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunization of children with asthma against pneumococcal infection with polysaccharide vaccine or combined immunization against pneumococcal infection and influenza reduced rate of asthma exacerbations and led to formation of immunity to vaccine strains of Streptococcus pneumoniae .
	manualset3
92628	7	399345	13	NULL	NULL	0	NULL	pneumococcal infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunization of children with asthma against pneumococcal infection with polysaccharide vaccine or combined immunization against pneumococcal infection and influenza reduced rate of asthma exacerbations and led to formation of immunity to vaccine strains of Streptococcus pneumoniae .
	manualset3
92629	8	399345	13	NULL	NULL	0	NULL	influenza	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunization of children with asthma against pneumococcal infection with polysaccharide vaccine or combined immunization against pneumococcal infection and influenza reduced rate of asthma exacerbations and led to formation of immunity to vaccine strains of Streptococcus pneumoniae .
	manualset3
92630	9	399345	13	NULL	NULL	0	NULL	rate of asthma exacerbations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunization of children with asthma against pneumococcal infection with polysaccharide vaccine or combined immunization against pneumococcal infection and influenza reduced rate of asthma exacerbations and led to formation of immunity to vaccine strains of Streptococcus pneumoniae .
	manualset3
92631	10	399345	13	NULL	NULL	0	NULL	formation of immunity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunization of children with asthma against pneumococcal infection with polysaccharide vaccine or combined immunization against pneumococcal infection and influenza reduced rate of asthma exacerbations and led to formation of immunity to vaccine strains of Streptococcus pneumoniae .
	manualset3
92632	11	399345	13	NULL	NULL	0	NULL	vaccine strains of Streptococcus pneumoniae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunization of children with asthma against pneumococcal infection with polysaccharide vaccine or combined immunization against pneumococcal infection and influenza reduced rate of asthma exacerbations and led to formation of immunity to vaccine strains of Streptococcus pneumoniae .
	manualset3
92633	1	399346	13	NULL	NULL	0	NULL	Immunization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunization with rgp96-tumor antigen complexes significantly inhibited B16 tumor growth compared with either rgp96 or tumor antigens alone and led to enhancement of tumor-specific T-cell activities , which was found similar to that of tumor tissue derived gp96 .
	manualset3
92634	2	399346	13	NULL	NULL	0	NULL	rgp96-tumor antigen complexes 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunization with rgp96-tumor antigen complexes significantly inhibited B16 tumor growth compared with either rgp96 or tumor antigens alone and led to enhancement of tumor-specific T-cell activities , which was found similar to that of tumor tissue derived gp96 .
	manualset3
92635	3	399346	13	NULL	NULL	0	NULL	 B16 tumor growth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunization with rgp96-tumor antigen complexes significantly inhibited B16 tumor growth compared with either rgp96 or tumor antigens alone and led to enhancement of tumor-specific T-cell activities , which was found similar to that of tumor tissue derived gp96 .
	manualset3
92636	4	399346	13	NULL	NULL	0	NULL	rgp96	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunization with rgp96-tumor antigen complexes significantly inhibited B16 tumor growth compared with either rgp96 or tumor antigens alone and led to enhancement of tumor-specific T-cell activities , which was found similar to that of tumor tissue derived gp96 .
	manualset3
92637	5	399346	13	NULL	NULL	0	NULL	 tumor antigens	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunization with rgp96-tumor antigen complexes significantly inhibited B16 tumor growth compared with either rgp96 or tumor antigens alone and led to enhancement of tumor-specific T-cell activities , which was found similar to that of tumor tissue derived gp96 .
	manualset3
92638	6	399346	13	NULL	NULL	0	NULL	 enhancement 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunization with rgp96-tumor antigen complexes significantly inhibited B16 tumor growth compared with either rgp96 or tumor antigens alone and led to enhancement of tumor-specific T-cell activities , which was found similar to that of tumor tissue derived gp96 .
	manualset3
92639	7	399346	13	NULL	NULL	0	NULL	tumor-specific T-cell activities 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunization with rgp96-tumor antigen complexes significantly inhibited B16 tumor growth compared with either rgp96 or tumor antigens alone and led to enhancement of tumor-specific T-cell activities , which was found similar to that of tumor tissue derived gp96 .
	manualset3
92641	8	399346	13	NULL	NULL	NULL	NULL	tumor tissue	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunization with rgp96-tumor antigen complexes significantly inhibited B16 tumor growth compared with either rgp96 or tumor antigens alone and led to enhancement of tumor-specific T-cell activities , which was found similar to that of tumor tissue derived gp96 .
	manualset3
92642	9	399346	13	NULL	NULL	NULL	NULL	gp96	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunization with rgp96-tumor antigen complexes significantly inhibited B16 tumor growth compared with either rgp96 or tumor antigens alone and led to enhancement of tumor-specific T-cell activities , which was found similar to that of tumor tissue derived gp96 .
	manualset3
92643	1	399347	13	NULL	NULL	0	NULL	Immunoarchitecture 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoarchitecture of eutopic remnants was indistinguishable from that of intact spleens and total nucleated cell counts remained proportional to weight .
	manualset3
92644	2	399347	13	NULL	NULL	0	NULL	eutopic remnants	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoarchitecture of eutopic remnants was indistinguishable from that of intact spleens and total nucleated cell counts remained proportional to weight .
	manualset3
92645	3	399347	13	NULL	NULL	0	NULL	intact spleens	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoarchitecture of eutopic remnants was indistinguishable from that of intact spleens and total nucleated cell counts remained proportional to weight .
	manualset3
92646	4	399347	13	NULL	NULL	0	NULL	total nucleated cell counts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoarchitecture of eutopic remnants was indistinguishable from that of intact spleens and total nucleated cell counts remained proportional to weight .
	manualset3
92647	5	399347	13	NULL	NULL	0	NULL	proportional to weight	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoarchitecture of eutopic remnants was indistinguishable from that of intact spleens and total nucleated cell counts remained proportional to weight .
	manualset3
92648	1	399348	13	NULL	NULL	0	NULL	Immunoassays 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoassays of the 1st and 2nd levels were investigated in patients with acute radiation disease 12-36 mos .
	manualset3
92649	2	399348	13	NULL	NULL	0	NULL	1st level	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoassays of the 1st and 2nd levels were investigated in patients with acute radiation disease 12-36 mos .
	manualset3
92650	3	399348	13	NULL	NULL	0	NULL	2nd level	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoassays of the 1st and 2nd levels were investigated in patients with acute radiation disease 12-36 mos .
	manualset3
92651	4	399348	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoassays of the 1st and 2nd levels were investigated in patients with acute radiation disease 12-36 mos .
	manualset3
92652	5	399348	13	NULL	NULL	0	NULL	acute radiation disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoassays of the 1st and 2nd levels were investigated in patients with acute radiation disease 12-36 mos .
	manualset3
92653	6	399348	13	NULL	NULL	0	NULL	12-36 mos	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoassays of the 1st and 2nd levels were investigated in patients with acute radiation disease 12-36 mos .
	manualset3
92654	1	399349	13	NULL	NULL	0	NULL	( 2 ) A short region	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( 2 ) A short region , largely uniform in length , which was located immediately 5 ' to each rTU .
	manualset3
92655	2	399349	13	NULL	NULL	0	NULL	 length	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( 2 ) A short region , largely uniform in length , which was located immediately 5 ' to each rTU .
	manualset3
92656	3	399349	13	NULL	NULL	0	NULL	5 ' to each rTU 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	( 2 ) A short region , largely uniform in length , which was located immediately 5 ' to each rTU .
	manualset3
92657	1	399350	13	NULL	NULL	0	NULL	 Anesthetic properties	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Anesthetic properties of a new inhibitor of glutaminergic transmission in the central nervous system , riluzole ) .
	manualset3
92658	2	399350	13	NULL	NULL	0	NULL	a new inhibitor of glutaminergic transmission	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Anesthetic properties of a new inhibitor of glutaminergic transmission in the central nervous system , riluzole ) .
	manualset3
92659	3	399350	13	NULL	NULL	0	NULL	 central nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Anesthetic properties of a new inhibitor of glutaminergic transmission in the central nervous system , riluzole ) .
	manualset3
92660	4	399350	13	NULL	NULL	NULL	NULL	riluzole	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Anesthetic properties of a new inhibitor of glutaminergic transmission in the central nervous system , riluzole ) .
	manualset3
92661	1	399351	13	NULL	NULL	0	NULL	Therapeutic effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Therapeutic effects and histological findings during administration of the cytostatic agent bleomycin ) .
	manualset3
92662	2	399351	13	NULL	NULL	0	NULL	histological findings 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Therapeutic effects and histological findings during administration of the cytostatic agent bleomycin ) .
	manualset3
92663	3	399351	13	NULL	NULL	0	NULL	 administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Therapeutic effects and histological findings during administration of the cytostatic agent bleomycin ) .
	manualset3
92664	4	399351	13	NULL	NULL	0	NULL	cytostatic agent bleomycin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Therapeutic effects and histological findings during administration of the cytostatic agent bleomycin ) .
	manualset3
92665	1	399352	13	NULL	NULL	0	NULL	Immunoblot analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoblot analysis demonstrated that type I - , IV - , and V-collagen-binding polypeptides ( CBPs ) were detected in the heated and unheated preparations from both Treponema denticola ATCC 33520 and T. socranskii subsp .
	manualset3
92666	2	399352	13	NULL	NULL	0	NULL	type I-collagen-binding polypeptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoblot analysis demonstrated that type I - , IV - , and V-collagen-binding polypeptides ( CBPs ) were detected in the heated and unheated preparations from both Treponema denticola ATCC 33520 and T. socranskii subsp .
	manualset3
92667	3	399352	13	NULL	NULL	0	NULL	type IV-collagen-binding polypeptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoblot analysis demonstrated that type I - , IV - , and V-collagen-binding polypeptides ( CBPs ) were detected in the heated and unheated preparations from both Treponema denticola ATCC 33520 and T. socranskii subsp .
	manualset3
92668	4	399352	13	NULL	NULL	0	NULL	type V-collagen-binding polypeptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoblot analysis demonstrated that type I - , IV - , and V-collagen-binding polypeptides ( CBPs ) were detected in the heated and unheated preparations from both Treponema denticola ATCC 33520 and T. socranskii subsp .
	manualset3
92669	5	399352	13	NULL	NULL	0	NULL	CBPs	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoblot analysis demonstrated that type I - , IV - , and V-collagen-binding polypeptides ( CBPs ) were detected in the heated and unheated preparations from both Treponema denticola ATCC 33520 and T. socranskii subsp .
	manualset3
92670	6	399352	13	NULL	NULL	0	NULL	 preparations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoblot analysis demonstrated that type I - , IV - , and V-collagen-binding polypeptides ( CBPs ) were detected in the heated and unheated preparations from both Treponema denticola ATCC 33520 and T. socranskii subsp .
	manualset3
92671	7	399352	13	NULL	NULL	0	NULL	Treponema denticola ATCC 33520 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoblot analysis demonstrated that type I - , IV - , and V-collagen-binding polypeptides ( CBPs ) were detected in the heated and unheated preparations from both Treponema denticola ATCC 33520 and T. socranskii subsp .
	manualset3
92672	8	399352	13	NULL	NULL	0	NULL	T. socranskii subsp	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoblot analysis demonstrated that type I - , IV - , and V-collagen-binding polypeptides ( CBPs ) were detected in the heated and unheated preparations from both Treponema denticola ATCC 33520 and T. socranskii subsp .
	manualset3
92673	1	399353	13	NULL	NULL	0	NULL	Immunoblot analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoblot analysis identifies the released pertussis toxin substrate as alpha subunits of Gi2 , Gi3 , and G ( o ) in the resolved supernatant .
	manualset3
92674	2	399353	13	NULL	NULL	0	NULL	pertussis toxin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoblot analysis identifies the released pertussis toxin substrate as alpha subunits of Gi2 , Gi3 , and G ( o ) in the resolved supernatant .
	manualset3
92675	3	399353	13	NULL	NULL	0	NULL	substrate	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoblot analysis identifies the released pertussis toxin substrate as alpha subunits of Gi2 , Gi3 , and G ( o ) in the resolved supernatant .
	manualset3
92676	4	399353	13	NULL	NULL	0	NULL	alpha subunit of Gi2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoblot analysis identifies the released pertussis toxin substrate as alpha subunits of Gi2 , Gi3 , and G ( o ) in the resolved supernatant .
	manualset3
92677	5	399353	13	NULL	NULL	0	NULL	 alpha subunits of Gi3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoblot analysis identifies the released pertussis toxin substrate as alpha subunits of Gi2 , Gi3 , and G ( o ) in the resolved supernatant .
	manualset3
92678	6	399353	13	NULL	NULL	0	NULL	alpha subunits of G ( o )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoblot analysis identifies the released pertussis toxin substrate as alpha subunits of Gi2 , Gi3 , and G ( o ) in the resolved supernatant .
	manualset3
92679	7	399353	13	NULL	NULL	NULL	NULL	 supernatant 	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunoblot analysis identifies the released pertussis toxin substrate as alpha subunits of Gi2 , Gi3 , and G ( o ) in the resolved supernatant .
	manualset3
92680	1	399354	13	NULL	NULL	0	NULL	Immunoblot 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoblot and RNA analysis revealed decreases in P450 2C11 apoprotein and its corresponding mRNA in liver from deficient rats that was prevented by inclusion of ATRA in the deficient diet .
	manualset3
92681	2	399354	13	NULL	NULL	0	NULL	RNA analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoblot and RNA analysis revealed decreases in P450 2C11 apoprotein and its corresponding mRNA in liver from deficient rats that was prevented by inclusion of ATRA in the deficient diet .
	manualset3
92682	3	399354	13	NULL	NULL	0	NULL	P450 2C11 apoprotein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoblot and RNA analysis revealed decreases in P450 2C11 apoprotein and its corresponding mRNA in liver from deficient rats that was prevented by inclusion of ATRA in the deficient diet .
	manualset3
92683	4	399354	13	NULL	NULL	0	NULL	mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoblot and RNA analysis revealed decreases in P450 2C11 apoprotein and its corresponding mRNA in liver from deficient rats that was prevented by inclusion of ATRA in the deficient diet .
	manualset3
92684	5	399354	13	NULL	NULL	0	NULL	liver 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoblot and RNA analysis revealed decreases in P450 2C11 apoprotein and its corresponding mRNA in liver from deficient rats that was prevented by inclusion of ATRA in the deficient diet .
	manualset3
92685	6	399354	13	NULL	NULL	0	NULL	deficient rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoblot and RNA analysis revealed decreases in P450 2C11 apoprotein and its corresponding mRNA in liver from deficient rats that was prevented by inclusion of ATRA in the deficient diet .
	manualset3
92686	7	399354	13	NULL	NULL	0	NULL	inclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoblot and RNA analysis revealed decreases in P450 2C11 apoprotein and its corresponding mRNA in liver from deficient rats that was prevented by inclusion of ATRA in the deficient diet .
	manualset3
92687	8	399354	13	NULL	NULL	0	NULL	ATRA	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoblot and RNA analysis revealed decreases in P450 2C11 apoprotein and its corresponding mRNA in liver from deficient rats that was prevented by inclusion of ATRA in the deficient diet .
	manualset3
92688	9	399354	13	NULL	NULL	0	NULL	deficient diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoblot and RNA analysis revealed decreases in P450 2C11 apoprotein and its corresponding mRNA in liver from deficient rats that was prevented by inclusion of ATRA in the deficient diet .
	manualset3
92690	1	399355	13	NULL	NULL	0	NULL	Immunoblotting	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoblotting of endogenous PKC phosphorylation confirmed PKC2 activation in response to IGF-II .
	manualset3
92691	2	399355	13	NULL	NULL	0	NULL	endogenous PKC phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoblotting of endogenous PKC phosphorylation confirmed PKC2 activation in response to IGF-II .
	manualset3
92692	3	399355	13	NULL	NULL	0	NULL	PKC2 activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoblotting of endogenous PKC phosphorylation confirmed PKC2 activation in response to IGF-II .
	manualset3
92693	4	399355	13	NULL	NULL	0	NULL	response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoblotting of endogenous PKC phosphorylation confirmed PKC2 activation in response to IGF-II .
	manualset3
92694	5	399355	13	NULL	NULL	0	NULL	IGF-II 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoblotting of endogenous PKC phosphorylation confirmed PKC2 activation in response to IGF-II .
	manualset3
92695	1	399356	13	NULL	NULL	0	NULL	Immunocharacterization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunocharacterization with beta-catenin , E-cadherin , cytokeratins ( AE1/AE3 ) , epithelial membrane antigen , S-100 protein , smooth muscle actin , and vimentin was also performed .
	manualset3
92696	2	399356	13	NULL	NULL	0	NULL	beta-catenin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunocharacterization with beta-catenin , E-cadherin , cytokeratins ( AE1/AE3 ) , epithelial membrane antigen , S-100 protein , smooth muscle actin , and vimentin was also performed .
	manualset3
92697	3	399356	13	NULL	NULL	0	NULL	E-cadherin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunocharacterization with beta-catenin , E-cadherin , cytokeratins ( AE1/AE3 ) , epithelial membrane antigen , S-100 protein , smooth muscle actin , and vimentin was also performed .
	manualset3
92698	4	399356	13	NULL	NULL	0	NULL	cytokeratins ( AE1/AE3 ) 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunocharacterization with beta-catenin , E-cadherin , cytokeratins ( AE1/AE3 ) , epithelial membrane antigen , S-100 protein , smooth muscle actin , and vimentin was also performed .
	manualset3
92699	5	399356	13	NULL	NULL	0	NULL	epithelial membrane antigen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunocharacterization with beta-catenin , E-cadherin , cytokeratins ( AE1/AE3 ) , epithelial membrane antigen , S-100 protein , smooth muscle actin , and vimentin was also performed .
	manualset3
92700	6	399356	13	NULL	NULL	0	NULL	S-100 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunocharacterization with beta-catenin , E-cadherin , cytokeratins ( AE1/AE3 ) , epithelial membrane antigen , S-100 protein , smooth muscle actin , and vimentin was also performed .
	manualset3
92701	7	399356	13	NULL	NULL	0	NULL	smooth muscle actin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunocharacterization with beta-catenin , E-cadherin , cytokeratins ( AE1/AE3 ) , epithelial membrane antigen , S-100 protein , smooth muscle actin , and vimentin was also performed .
	manualset3
92702	8	399356	13	NULL	NULL	0	NULL	vimentin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunocharacterization with beta-catenin , E-cadherin , cytokeratins ( AE1/AE3 ) , epithelial membrane antigen , S-100 protein , smooth muscle actin , and vimentin was also performed .
	manualset3
92703	1	399357	13	NULL	NULL	0	NULL	Immunochemical studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunochemical studies of heat-shock protein 80 of Histoplasma capsulatum .
	manualset3
92704	2	399357	13	NULL	NULL	0	NULL	heat-shock protein 80	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunochemical studies of heat-shock protein 80 of Histoplasma capsulatum .
	manualset3
92705	3	399357	13	NULL	NULL	0	NULL	Histoplasma capsulatum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunochemical studies of heat-shock protein 80 of Histoplasma capsulatum .
	manualset3
92706	1	399358	13	NULL	NULL	0	NULL	Immunochemical studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunochemical studies with monoclonal antibodies against rat liver cytochrome P450 isoenzymes of the gene families 1A , 2B , 3A , and 4A confirmed that bromopropylate is a phenobarbitone-type inducer in the mouse liver .
	manualset3
92707	2	399358	13	NULL	NULL	0	NULL	monoclonal antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunochemical studies with monoclonal antibodies against rat liver cytochrome P450 isoenzymes of the gene families 1A , 2B , 3A , and 4A confirmed that bromopropylate is a phenobarbitone-type inducer in the mouse liver .
	manualset3
92708	3	399358	13	NULL	NULL	0	NULL	rat liver cytochrome P450 isoenzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunochemical studies with monoclonal antibodies against rat liver cytochrome P450 isoenzymes of the gene families 1A , 2B , 3A , and 4A confirmed that bromopropylate is a phenobarbitone-type inducer in the mouse liver .
	manualset3
92709	4	399358	13	NULL	NULL	0	NULL	gene families 1A	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunochemical studies with monoclonal antibodies against rat liver cytochrome P450 isoenzymes of the gene families 1A , 2B , 3A , and 4A confirmed that bromopropylate is a phenobarbitone-type inducer in the mouse liver .
	manualset3
92710	5	399358	13	NULL	NULL	0	NULL	gene families 2B	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunochemical studies with monoclonal antibodies against rat liver cytochrome P450 isoenzymes of the gene families 1A , 2B , 3A , and 4A confirmed that bromopropylate is a phenobarbitone-type inducer in the mouse liver .
	manualset3
92711	6	399358	13	NULL	NULL	0	NULL	gene families 3A	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunochemical studies with monoclonal antibodies against rat liver cytochrome P450 isoenzymes of the gene families 1A , 2B , 3A , and 4A confirmed that bromopropylate is a phenobarbitone-type inducer in the mouse liver .
	manualset3
92712	7	399358	13	NULL	NULL	0	NULL	gene families 4A	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunochemical studies with monoclonal antibodies against rat liver cytochrome P450 isoenzymes of the gene families 1A , 2B , 3A , and 4A confirmed that bromopropylate is a phenobarbitone-type inducer in the mouse liver .
	manualset3
92713	8	399358	13	NULL	NULL	0	NULL	bromopropylate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunochemical studies with monoclonal antibodies against rat liver cytochrome P450 isoenzymes of the gene families 1A , 2B , 3A , and 4A confirmed that bromopropylate is a phenobarbitone-type inducer in the mouse liver .
	manualset3
92714	9	399358	13	NULL	NULL	0	NULL	phenobarbitone-type inducer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunochemical studies with monoclonal antibodies against rat liver cytochrome P450 isoenzymes of the gene families 1A , 2B , 3A , and 4A confirmed that bromopropylate is a phenobarbitone-type inducer in the mouse liver .
	manualset3
92715	10	399358	13	NULL	NULL	0	NULL	mouse liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunochemical studies with monoclonal antibodies against rat liver cytochrome P450 isoenzymes of the gene families 1A , 2B , 3A , and 4A confirmed that bromopropylate is a phenobarbitone-type inducer in the mouse liver .
	manualset3
92716	1	399359	13	NULL	NULL	0	NULL	Therapeutic management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Therapeutic management of peptic ulcer bleeding ) .
	manualset3
92717	2	399359	13	NULL	NULL	0	NULL	peptic ulcer bleeding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Therapeutic management of peptic ulcer bleeding ) .
	manualset3
92718	1	399360	13	NULL	NULL	0	NULL	Immunocytochemical localization studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunocytochemical localization studies found estrogen receptor alpha ( ERalpha ) and estrogen receptor beta ( ERbeta ) in cortical neurons and glia .
	manualset3
92719	2	399360	13	NULL	NULL	0	NULL	estrogen receptor alpha ( ERalpha ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunocytochemical localization studies found estrogen receptor alpha ( ERalpha ) and estrogen receptor beta ( ERbeta ) in cortical neurons and glia .
	manualset3
92720	3	399360	13	NULL	NULL	0	NULL	estrogen receptor beta ( ERbeta )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunocytochemical localization studies found estrogen receptor alpha ( ERalpha ) and estrogen receptor beta ( ERbeta ) in cortical neurons and glia .
	manualset3
92721	4	399360	13	NULL	NULL	0	NULL	cortical neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunocytochemical localization studies found estrogen receptor alpha ( ERalpha ) and estrogen receptor beta ( ERbeta ) in cortical neurons and glia .
	manualset3
92722	5	399360	13	NULL	NULL	0	NULL	 glia	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunocytochemical localization studies found estrogen receptor alpha ( ERalpha ) and estrogen receptor beta ( ERbeta ) in cortical neurons and glia .
	manualset3
92723	1	399361	13	NULL	NULL	0	NULL	Immunocytochemistry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunocytochemistry of the taurine biosynthesis enzyme , cysteine sulfinate decarboxylase , in the cerebellum : evidence for a glial localization .
	manualset3
92724	2	399361	13	NULL	NULL	0	NULL	taurine biosynthesis enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunocytochemistry of the taurine biosynthesis enzyme , cysteine sulfinate decarboxylase , in the cerebellum : evidence for a glial localization .
	manualset3
92725	3	399361	13	NULL	NULL	0	NULL	cysteine sulfinate decarboxylase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunocytochemistry of the taurine biosynthesis enzyme , cysteine sulfinate decarboxylase , in the cerebellum : evidence for a glial localization .
	manualset3
92726	4	399361	13	NULL	NULL	0	NULL	cerebellum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunocytochemistry of the taurine biosynthesis enzyme , cysteine sulfinate decarboxylase , in the cerebellum : evidence for a glial localization .
	manualset3
92728	5	399361	13	NULL	NULL	NULL	NULL	glial localization	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunocytochemistry of the taurine biosynthesis enzyme , cysteine sulfinate decarboxylase , in the cerebellum : evidence for a glial localization .
	manualset3
94210	6	399361	13	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunocytochemistry of the taurine biosynthesis enzyme , cysteine sulfinate decarboxylase , in the cerebellum : evidence for a glial localization .
	manualset3
92729	1	399362	13	NULL	NULL	0	NULL	Immunocytochemistry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunocytochemistry showed that the distribution of beacon protein followed that of beacon mRNA .
	manualset3
92730	2	399362	13	NULL	NULL	0	NULL	 distribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunocytochemistry showed that the distribution of beacon protein followed that of beacon mRNA .
	manualset3
92731	3	399362	13	NULL	NULL	0	NULL	beacon protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunocytochemistry showed that the distribution of beacon protein followed that of beacon mRNA .
	manualset3
92732	4	399362	13	NULL	NULL	0	NULL	beacon mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunocytochemistry showed that the distribution of beacon protein followed that of beacon mRNA .
	manualset3
92733	1	399363	13	NULL	NULL	0	NULL	Immunoelectron microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoelectron microscopy demonstrated that CgA and SgIII were specifically colocalized in large secretory granules in male rat gonadotropes , which possess large-type and small-type granules .
	manualset3
92734	2	399363	13	NULL	NULL	0	NULL	CgA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoelectron microscopy demonstrated that CgA and SgIII were specifically colocalized in large secretory granules in male rat gonadotropes , which possess large-type and small-type granules .
	manualset3
92735	3	399363	13	NULL	NULL	0	NULL	 SgIII	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoelectron microscopy demonstrated that CgA and SgIII were specifically colocalized in large secretory granules in male rat gonadotropes , which possess large-type and small-type granules .
	manualset3
92736	4	399363	13	NULL	NULL	0	NULL	large secretory granules	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoelectron microscopy demonstrated that CgA and SgIII were specifically colocalized in large secretory granules in male rat gonadotropes , which possess large-type and small-type granules .
	manualset3
92737	5	399363	13	NULL	NULL	0	NULL	male rat gonadotropes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoelectron microscopy demonstrated that CgA and SgIII were specifically colocalized in large secretory granules in male rat gonadotropes , which possess large-type and small-type granules .
	manualset3
92738	6	399363	13	NULL	NULL	0	NULL	large-type granules	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoelectron microscopy demonstrated that CgA and SgIII were specifically colocalized in large secretory granules in male rat gonadotropes , which possess large-type and small-type granules .
	manualset3
92739	7	399363	13	NULL	NULL	0	NULL	small-type granules	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoelectron microscopy demonstrated that CgA and SgIII were specifically colocalized in large secretory granules in male rat gonadotropes , which possess large-type and small-type granules .
	manualset3
92740	1	399364	13	NULL	NULL	0	NULL	Immunofluorescence 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence and in vitro ( ( 35 ) S ) GTPgammaS autoradiography of rat tissue sections containing the PBN revealed the presence of cannabinoid receptors and their functional capability to couple to their G-proteins after incubation with the endocannabinoid 2-arachidonoyl glycerol ( 2-AG ) .
	manualset3
92741	2	399364	13	NULL	NULL	NULL	NULL	 in vitro ( ( 35 ) S ) GTPgammaS autoradiography	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunofluorescence and in vitro ( ( 35 ) S ) GTPgammaS autoradiography of rat tissue sections containing the PBN revealed the presence of cannabinoid receptors and their functional capability to couple to their G-proteins after incubation with the endocannabinoid 2-arachidonoyl glycerol ( 2-AG ) .
	manualset3
92742	3	399364	13	NULL	NULL	0	NULL	rat tissue sections	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence and in vitro ( ( 35 ) S ) GTPgammaS autoradiography of rat tissue sections containing the PBN revealed the presence of cannabinoid receptors and their functional capability to couple to their G-proteins after incubation with the endocannabinoid 2-arachidonoyl glycerol ( 2-AG ) .
	manualset3
92743	4	399364	13	NULL	NULL	0	NULL	PBN 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence and in vitro ( ( 35 ) S ) GTPgammaS autoradiography of rat tissue sections containing the PBN revealed the presence of cannabinoid receptors and their functional capability to couple to their G-proteins after incubation with the endocannabinoid 2-arachidonoyl glycerol ( 2-AG ) .
	manualset3
92744	5	399364	13	NULL	NULL	0	NULL	cannabinoid receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence and in vitro ( ( 35 ) S ) GTPgammaS autoradiography of rat tissue sections containing the PBN revealed the presence of cannabinoid receptors and their functional capability to couple to their G-proteins after incubation with the endocannabinoid 2-arachidonoyl glycerol ( 2-AG ) .
	manualset3
92745	6	399364	13	NULL	NULL	0	NULL	 functional capability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence and in vitro ( ( 35 ) S ) GTPgammaS autoradiography of rat tissue sections containing the PBN revealed the presence of cannabinoid receptors and their functional capability to couple to their G-proteins after incubation with the endocannabinoid 2-arachidonoyl glycerol ( 2-AG ) .
	manualset3
92746	7	399364	13	NULL	NULL	0	NULL	G-proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence and in vitro ( ( 35 ) S ) GTPgammaS autoradiography of rat tissue sections containing the PBN revealed the presence of cannabinoid receptors and their functional capability to couple to their G-proteins after incubation with the endocannabinoid 2-arachidonoyl glycerol ( 2-AG ) .
	manualset3
92747	8	399364	13	NULL	NULL	0	NULL	incubation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence and in vitro ( ( 35 ) S ) GTPgammaS autoradiography of rat tissue sections containing the PBN revealed the presence of cannabinoid receptors and their functional capability to couple to their G-proteins after incubation with the endocannabinoid 2-arachidonoyl glycerol ( 2-AG ) .
	manualset3
92748	9	399364	13	NULL	NULL	0	NULL	endocannabinoid 2-arachidonoyl glycerol ( 2-AG )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence and in vitro ( ( 35 ) S ) GTPgammaS autoradiography of rat tissue sections containing the PBN revealed the presence of cannabinoid receptors and their functional capability to couple to their G-proteins after incubation with the endocannabinoid 2-arachidonoyl glycerol ( 2-AG ) .
	manualset3
94211	5	399364	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence and in vitro ( ( 35 ) S ) GTPgammaS autoradiography of rat tissue sections containing the PBN revealed the presence of cannabinoid receptors and their functional capability to couple to their G-proteins after incubation with the endocannabinoid 2-arachidonoyl glycerol ( 2-AG ) .
	manualset3
92749	1	399365	13	NULL	NULL	0	NULL	Immunofluorescence 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence demonstrated that HUVEC expressed AHR and ER but lacked ER and the involvement of AHR and ER on the effects of PCB126 was examined by the addition of AHR and ER antagonists .
	manualset3
92750	2	399365	13	NULL	NULL	0	NULL	HUVEC 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence demonstrated that HUVEC expressed AHR and ER but lacked ER and the involvement of AHR and ER on the effects of PCB126 was examined by the addition of AHR and ER antagonists .
	manualset3
92751	3	399365	13	NULL	NULL	0	NULL	AHR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence demonstrated that HUVEC expressed AHR and ER but lacked ER and the involvement of AHR and ER on the effects of PCB126 was examined by the addition of AHR and ER antagonists .
	manualset3
92752	4	399365	13	NULL	NULL	0	NULL	 ER	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence demonstrated that HUVEC expressed AHR and ER but lacked ER and the involvement of AHR and ER on the effects of PCB126 was examined by the addition of AHR and ER antagonists .
	manualset3
92753	5	399365	13	NULL	NULL	0	NULL	ER 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence demonstrated that HUVEC expressed AHR and ER but lacked ER and the involvement of AHR and ER on the effects of PCB126 was examined by the addition of AHR and ER antagonists .
	manualset3
92754	6	399365	13	NULL	NULL	0	NULL	involvement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence demonstrated that HUVEC expressed AHR and ER but lacked ER and the involvement of AHR and ER on the effects of PCB126 was examined by the addition of AHR and ER antagonists .
	manualset3
92755	7	399365	13	NULL	NULL	0	NULL	AHR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence demonstrated that HUVEC expressed AHR and ER but lacked ER and the involvement of AHR and ER on the effects of PCB126 was examined by the addition of AHR and ER antagonists .
	manualset3
92756	8	399365	13	NULL	NULL	0	NULL	ER	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence demonstrated that HUVEC expressed AHR and ER but lacked ER and the involvement of AHR and ER on the effects of PCB126 was examined by the addition of AHR and ER antagonists .
	manualset3
92757	9	399365	13	NULL	NULL	0	NULL	PCB126	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence demonstrated that HUVEC expressed AHR and ER but lacked ER and the involvement of AHR and ER on the effects of PCB126 was examined by the addition of AHR and ER antagonists .
	manualset3
92759	10	399365	13	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence demonstrated that HUVEC expressed AHR and ER but lacked ER and the involvement of AHR and ER on the effects of PCB126 was examined by the addition of AHR and ER antagonists .
	manualset3
92760	11	399365	13	NULL	NULL	0	NULL	AHR antagonists 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence demonstrated that HUVEC expressed AHR and ER but lacked ER and the involvement of AHR and ER on the effects of PCB126 was examined by the addition of AHR and ER antagonists .
	manualset3
92761	12	399365	13	NULL	NULL	0	NULL	ER antagonists	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence demonstrated that HUVEC expressed AHR and ER but lacked ER and the involvement of AHR and ER on the effects of PCB126 was examined by the addition of AHR and ER antagonists .
	manualset3
92762	1	399366	13	NULL	NULL	0	NULL	Immunofluorescence 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence observations show that TrkA-GFP is found mainly in cell surface membrane ruffles and in endosomes .
	manualset3
92763	2	399366	13	NULL	NULL	0	NULL	 observations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence observations show that TrkA-GFP is found mainly in cell surface membrane ruffles and in endosomes .
	manualset3
92764	3	399366	13	NULL	NULL	0	NULL	 TrkA-GFP 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence observations show that TrkA-GFP is found mainly in cell surface membrane ruffles and in endosomes .
	manualset3
92765	4	399366	13	NULL	NULL	0	NULL	cell surface membrane ruffles 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence observations show that TrkA-GFP is found mainly in cell surface membrane ruffles and in endosomes .
	manualset3
92766	5	399366	13	NULL	NULL	0	NULL	endosomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence observations show that TrkA-GFP is found mainly in cell surface membrane ruffles and in endosomes .
	manualset3
92767	1	399367	13	NULL	NULL	0	NULL	Immunofluorescence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence of sarcomeric a-actin was enhanced and its expression increased dose - and time-dependently in T3-treated cultured heart myocytes .
	manualset3
92768	2	399367	13	NULL	NULL	0	NULL	 sarcomeric a-actin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence of sarcomeric a-actin was enhanced and its expression increased dose - and time-dependently in T3-treated cultured heart myocytes .
	manualset3
92769	3	399367	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence of sarcomeric a-actin was enhanced and its expression increased dose - and time-dependently in T3-treated cultured heart myocytes .
	manualset3
92770	4	399367	13	NULL	NULL	0	NULL	dose	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence of sarcomeric a-actin was enhanced and its expression increased dose - and time-dependently in T3-treated cultured heart myocytes .
	manualset3
92771	5	399367	13	NULL	NULL	0	NULL	T3-treated cultured heart myocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunofluorescence of sarcomeric a-actin was enhanced and its expression increased dose - and time-dependently in T3-treated cultured heart myocytes .
	manualset3
92772	1	399368	13	NULL	NULL	NULL	NULL	Immunogenicity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunogenicity of Bacteroides isolated from mice : relationship between immunogenicity and cell wall antigens .
	manualset3
92773	2	399368	13	NULL	NULL	0	NULL	Bacteroides	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunogenicity of Bacteroides isolated from mice : relationship between immunogenicity and cell wall antigens .
	manualset3
92774	3	399368	13	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunogenicity of Bacteroides isolated from mice : relationship between immunogenicity and cell wall antigens .
	manualset3
92775	4	399368	13	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunogenicity of Bacteroides isolated from mice : relationship between immunogenicity and cell wall antigens .
	manualset3
92776	5	399368	13	NULL	NULL	NULL	NULL	immunogenicity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunogenicity of Bacteroides isolated from mice : relationship between immunogenicity and cell wall antigens .
	manualset3
92777	6	399368	13	NULL	NULL	0	NULL	cell wall antigens	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunogenicity of Bacteroides isolated from mice : relationship between immunogenicity and cell wall antigens .
	manualset3
92778	1	399369	13	NULL	NULL	NULL	NULL	Immunogenicity 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunogenicity of well-characterized synthetic Plasmodium falciparum multiple antigen peptide conjugates .
	manualset3
92779	2	399369	13	NULL	NULL	0	NULL	 synthetic Plasmodium falciparum multiple antigen peptide conjugates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunogenicity of well-characterized synthetic Plasmodium falciparum multiple antigen peptide conjugates .
	manualset3
92780	1	399370	13	NULL	NULL	0	NULL	Immunoglobulin E antibodies 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoglobulin E antibodies to ingested cereal flour components : studies with sera from subjects with asthma and eczema .
	manualset3
92781	2	399370	13	NULL	NULL	0	NULL	cereal flour components	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoglobulin E antibodies to ingested cereal flour components : studies with sera from subjects with asthma and eczema .
	manualset3
92782	3	399370	13	NULL	NULL	0	NULL	sera	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoglobulin E antibodies to ingested cereal flour components : studies with sera from subjects with asthma and eczema .
	manualset3
92783	5	399370	13	NULL	NULL	NULL	NULL	subjects with asthma	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunoglobulin E antibodies to ingested cereal flour components : studies with sera from subjects with asthma and eczema .
	manualset3
92784	6	399370	13	NULL	NULL	NULL	NULL	subjects with eczema	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunoglobulin E antibodies to ingested cereal flour components : studies with sera from subjects with asthma and eczema .
	manualset3
94213	4	399370	13	NULL	NULL	0	NULL	studies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoglobulin E antibodies to ingested cereal flour components : studies with sera from subjects with asthma and eczema .
	manualset3
92794	1	399371	13	NULL	NULL	NULL	NULL	Immunoglobulin G	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunoglobulin G may be prepared by different methods for intravenous infusion and administered as replacement therapy for hypogammaglobulinemia .
	manualset3
92795	2	399371	13	NULL	NULL	0	NULL	different methods	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoglobulin G may be prepared by different methods for intravenous infusion and administered as replacement therapy for hypogammaglobulinemia .
	manualset3
92796	3	399371	13	NULL	NULL	0	NULL	intravenous infusion 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoglobulin G may be prepared by different methods for intravenous infusion and administered as replacement therapy for hypogammaglobulinemia .
	manualset3
92797	4	399371	13	NULL	NULL	0	NULL	replacement therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoglobulin G may be prepared by different methods for intravenous infusion and administered as replacement therapy for hypogammaglobulinemia .
	manualset3
92799	5	399371	13	NULL	NULL	0	NULL	hypogammaglobulinemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoglobulin G may be prepared by different methods for intravenous infusion and administered as replacement therapy for hypogammaglobulinemia .
	manualset3
92802	1	399372	13	NULL	NULL	0	NULL	Immunoglobulin G4-related systemic disease ( IgG4-RSD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoglobulin G4-related systemic disease ( IgG4-RSD ) is a recently defined emerging entity characterized by a diffuse or mass forming inflammatory reaction rich in IgG4-positive plasma cells associated with fibrosclerosis and obliterative phlebitis .
	manualset3
92803	2	399372	13	NULL	NULL	0	NULL	emerging entity	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoglobulin G4-related systemic disease ( IgG4-RSD ) is a recently defined emerging entity characterized by a diffuse or mass forming inflammatory reaction rich in IgG4-positive plasma cells associated with fibrosclerosis and obliterative phlebitis .
	manualset3
92804	3	399372	13	NULL	NULL	0	NULL	diffuse or mass forming inflammatory reaction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoglobulin G4-related systemic disease ( IgG4-RSD ) is a recently defined emerging entity characterized by a diffuse or mass forming inflammatory reaction rich in IgG4-positive plasma cells associated with fibrosclerosis and obliterative phlebitis .
	manualset3
92805	4	399372	13	NULL	NULL	0	NULL	IgG4-positive plasma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoglobulin G4-related systemic disease ( IgG4-RSD ) is a recently defined emerging entity characterized by a diffuse or mass forming inflammatory reaction rich in IgG4-positive plasma cells associated with fibrosclerosis and obliterative phlebitis .
	manualset3
92806	5	399372	13	NULL	NULL	0	NULL	fibrosclerosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoglobulin G4-related systemic disease ( IgG4-RSD ) is a recently defined emerging entity characterized by a diffuse or mass forming inflammatory reaction rich in IgG4-positive plasma cells associated with fibrosclerosis and obliterative phlebitis .
	manualset3
92808	6	399372	13	NULL	NULL	0	NULL	obliterative phlebitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoglobulin G4-related systemic disease ( IgG4-RSD ) is a recently defined emerging entity characterized by a diffuse or mass forming inflammatory reaction rich in IgG4-positive plasma cells associated with fibrosclerosis and obliterative phlebitis .
	manualset3
92811	1	399373	13	NULL	NULL	0	NULL	Immunohistochemical study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical , electrophysiological , and electron microscopical study of rat fungiform taste buds after regeneration of chorda tympani through the non-gustatory lingual nerve .
	manualset3
92812	2	399373	13	NULL	NULL	0	NULL	electrophysiological study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical , electrophysiological , and electron microscopical study of rat fungiform taste buds after regeneration of chorda tympani through the non-gustatory lingual nerve .
	manualset3
92813	3	399373	13	NULL	NULL	0	NULL	electron microscopical study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical , electrophysiological , and electron microscopical study of rat fungiform taste buds after regeneration of chorda tympani through the non-gustatory lingual nerve .
	manualset3
92814	4	399373	13	NULL	NULL	0	NULL	rat fungiform taste buds	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical , electrophysiological , and electron microscopical study of rat fungiform taste buds after regeneration of chorda tympani through the non-gustatory lingual nerve .
	manualset3
92815	5	399373	13	NULL	NULL	0	NULL	regeneration 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical , electrophysiological , and electron microscopical study of rat fungiform taste buds after regeneration of chorda tympani through the non-gustatory lingual nerve .
	manualset3
92816	6	399373	13	NULL	NULL	0	NULL	chorda tympani 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical , electrophysiological , and electron microscopical study of rat fungiform taste buds after regeneration of chorda tympani through the non-gustatory lingual nerve .
	manualset3
92817	7	399373	13	NULL	NULL	0	NULL	non-gustatory lingual nerve	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical , electrophysiological , and electron microscopical study of rat fungiform taste buds after regeneration of chorda tympani through the non-gustatory lingual nerve .
	manualset3
92818	1	399374	13	NULL	NULL	0	NULL	Immunohistochemical analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical analyses were performed on multiple sections of ML specimens to evaluate Pgp expression .
	manualset3
92819	2	399374	13	NULL	NULL	0	NULL	multiple sections of ML specimens	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical analyses were performed on multiple sections of ML specimens to evaluate Pgp expression .
	manualset3
92820	3	399374	13	NULL	NULL	0	NULL	Pgp expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical analyses were performed on multiple sections of ML specimens to evaluate Pgp expression .
	manualset3
92822	1	399375	13	NULL	NULL	0	NULL	Immunohistochemical analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical analysis in 172 cases of breast tissues showed that the positive rate of CacyBP protein expression in normal breast tissues ( NBT ) ( 89.3 % ) was higher than that in invasive ductal carcinoma ( IDC ) ( 56.1 % ) ( P & lt ; 0.05 ) .
	manualset3
92823	2	399375	13	NULL	NULL	0	NULL	172 cases	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical analysis in 172 cases of breast tissues showed that the positive rate of CacyBP protein expression in normal breast tissues ( NBT ) ( 89.3 % ) was higher than that in invasive ductal carcinoma ( IDC ) ( 56.1 % ) ( P & lt ; 0.05 ) .
	manualset3
92824	3	399375	13	NULL	NULL	0	NULL	breast tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical analysis in 172 cases of breast tissues showed that the positive rate of CacyBP protein expression in normal breast tissues ( NBT ) ( 89.3 % ) was higher than that in invasive ductal carcinoma ( IDC ) ( 56.1 % ) ( P & lt ; 0.05 ) .
	manualset3
92825	4	399375	13	NULL	NULL	0	NULL	positive rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical analysis in 172 cases of breast tissues showed that the positive rate of CacyBP protein expression in normal breast tissues ( NBT ) ( 89.3 % ) was higher than that in invasive ductal carcinoma ( IDC ) ( 56.1 % ) ( P & lt ; 0.05 ) .
	manualset3
92826	5	399375	13	NULL	NULL	0	NULL	CacyBP protein expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical analysis in 172 cases of breast tissues showed that the positive rate of CacyBP protein expression in normal breast tissues ( NBT ) ( 89.3 % ) was higher than that in invasive ductal carcinoma ( IDC ) ( 56.1 % ) ( P & lt ; 0.05 ) .
	manualset3
92827	6	399375	13	NULL	NULL	0	NULL	normal breast tissues ( NBT ) 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical analysis in 172 cases of breast tissues showed that the positive rate of CacyBP protein expression in normal breast tissues ( NBT ) ( 89.3 % ) was higher than that in invasive ductal carcinoma ( IDC ) ( 56.1 % ) ( P & lt ; 0.05 ) .
	manualset3
92828	7	399375	13	NULL	NULL	0	NULL	 89.3 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical analysis in 172 cases of breast tissues showed that the positive rate of CacyBP protein expression in normal breast tissues ( NBT ) ( 89.3 % ) was higher than that in invasive ductal carcinoma ( IDC ) ( 56.1 % ) ( P & lt ; 0.05 ) .
	manualset3
92829	8	399375	13	NULL	NULL	0	NULL	invasive ductal carcinoma ( IDC )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical analysis in 172 cases of breast tissues showed that the positive rate of CacyBP protein expression in normal breast tissues ( NBT ) ( 89.3 % ) was higher than that in invasive ductal carcinoma ( IDC ) ( 56.1 % ) ( P & lt ; 0.05 ) .
	manualset3
92830	9	399375	13	NULL	NULL	0	NULL	( 56.1 % ) ( P & lt ; 0.05 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical analysis in 172 cases of breast tissues showed that the positive rate of CacyBP protein expression in normal breast tissues ( NBT ) ( 89.3 % ) was higher than that in invasive ductal carcinoma ( IDC ) ( 56.1 % ) ( P & lt ; 0.05 ) .
	manualset3
92831	1	399376	13	NULL	NULL	0	NULL	Immunohistochemical analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical analysis of 14-3-3 sigma and related proteins in hyperplastic and neoplastic breast lesions , with particular reference to early carcinogenesis .
	manualset3
92832	2	399376	13	NULL	NULL	0	NULL	14-3-3 sigma	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical analysis of 14-3-3 sigma and related proteins in hyperplastic and neoplastic breast lesions , with particular reference to early carcinogenesis .
	manualset3
92833	3	399376	13	NULL	NULL	0	NULL	 related proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical analysis of 14-3-3 sigma and related proteins in hyperplastic and neoplastic breast lesions , with particular reference to early carcinogenesis .
	manualset3
92834	4	399376	13	NULL	NULL	0	NULL	hyperplastic breast lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical analysis of 14-3-3 sigma and related proteins in hyperplastic and neoplastic breast lesions , with particular reference to early carcinogenesis .
	manualset3
92835	5	399376	13	NULL	NULL	0	NULL	neoplastic breast lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical analysis of 14-3-3 sigma and related proteins in hyperplastic and neoplastic breast lesions , with particular reference to early carcinogenesis .
	manualset3
92836	7	399376	13	NULL	NULL	NULL	NULL	 carcinogenesis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunohistochemical analysis of 14-3-3 sigma and related proteins in hyperplastic and neoplastic breast lesions , with particular reference to early carcinogenesis .
	manualset3
94214	6	399376	13	NULL	NULL	0	NULL	reference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical analysis of 14-3-3 sigma and related proteins in hyperplastic and neoplastic breast lesions , with particular reference to early carcinogenesis .
	manualset3
92837	1	399377	13	NULL	NULL	0	NULL	Immunohistochemical analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical analysis revealed a strong nuclear Snail staining in mock-transfected cells compared with a significantly reduced nuclear staining and translocation to the cytoplasm in P-cadherin-overexpressing cells .
	manualset3
92838	2	399377	13	NULL	NULL	0	NULL	 strong nuclear Snail staining	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical analysis revealed a strong nuclear Snail staining in mock-transfected cells compared with a significantly reduced nuclear staining and translocation to the cytoplasm in P-cadherin-overexpressing cells .
	manualset3
92839	3	399377	13	NULL	NULL	0	NULL	 mock-transfected cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical analysis revealed a strong nuclear Snail staining in mock-transfected cells compared with a significantly reduced nuclear staining and translocation to the cytoplasm in P-cadherin-overexpressing cells .
	manualset3
92840	4	399377	13	NULL	NULL	0	NULL	nuclear staining	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical analysis revealed a strong nuclear Snail staining in mock-transfected cells compared with a significantly reduced nuclear staining and translocation to the cytoplasm in P-cadherin-overexpressing cells .
	manualset3
92841	5	399377	13	NULL	NULL	0	NULL	translocation to the cytoplasm 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical analysis revealed a strong nuclear Snail staining in mock-transfected cells compared with a significantly reduced nuclear staining and translocation to the cytoplasm in P-cadherin-overexpressing cells .
	manualset3
92842	6	399377	13	NULL	NULL	0	NULL	P-cadherin-overexpressing cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical analysis revealed a strong nuclear Snail staining in mock-transfected cells compared with a significantly reduced nuclear staining and translocation to the cytoplasm in P-cadherin-overexpressing cells .
	manualset3
92843	1	399378	13	NULL	NULL	0	NULL	Therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Therapy and survival in thyroid tumors ) .
	manualset3
92844	2	399378	13	NULL	NULL	0	NULL	survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Therapy and survival in thyroid tumors ) .
	manualset3
92845	3	399378	13	NULL	NULL	0	NULL	thyroid tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Therapy and survival in thyroid tumors ) .
	manualset3
92846	1	399379	13	NULL	NULL	0	NULL	Immunohistochemical detection 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical detection of gastric mucin in normal and disease states .
	manualset3
92847	2	399379	13	NULL	NULL	0	NULL	gastric mucin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical detection of gastric mucin in normal and disease states .
	manualset3
92848	3	399379	13	NULL	NULL	0	NULL	normal states	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical detection of gastric mucin in normal and disease states .
	manualset3
92849	4	399379	13	NULL	NULL	0	NULL	disease states	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical detection of gastric mucin in normal and disease states .
	manualset3
92850	1	399380	13	NULL	NULL	0	NULL	Immunohistochemical detection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical detection of the protein , Fos , was used to identify neurons in the brain activated following a volume load in conscious rabbits with doxorubicin-induced congestive cardiomyopathy .
	manualset3
92851	2	399380	13	NULL	NULL	0	NULL	 protein , Fos	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical detection of the protein , Fos , was used to identify neurons in the brain activated following a volume load in conscious rabbits with doxorubicin-induced congestive cardiomyopathy .
	manualset3
92852	3	399380	13	NULL	NULL	0	NULL	neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical detection of the protein , Fos , was used to identify neurons in the brain activated following a volume load in conscious rabbits with doxorubicin-induced congestive cardiomyopathy .
	manualset3
92853	4	399380	13	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical detection of the protein , Fos , was used to identify neurons in the brain activated following a volume load in conscious rabbits with doxorubicin-induced congestive cardiomyopathy .
	manualset3
92854	5	399380	13	NULL	NULL	0	NULL	 volume load	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical detection of the protein , Fos , was used to identify neurons in the brain activated following a volume load in conscious rabbits with doxorubicin-induced congestive cardiomyopathy .
	manualset3
92855	6	399380	13	NULL	NULL	0	NULL	conscious rabbits	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical detection of the protein , Fos , was used to identify neurons in the brain activated following a volume load in conscious rabbits with doxorubicin-induced congestive cardiomyopathy .
	manualset3
92856	7	399380	13	NULL	NULL	0	NULL	doxorubicin-induced congestive cardiomyopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical detection of the protein , Fos , was used to identify neurons in the brain activated following a volume load in conscious rabbits with doxorubicin-induced congestive cardiomyopathy .
	manualset3
92857	1	399381	13	NULL	NULL	0	NULL	Immunohistochemical staining 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical staining for estrogen receptors in the endometrium was positive in all but one treated gilts , and negative to weakly positive in control gilts .
	manualset3
92858	2	399381	13	NULL	NULL	0	NULL	estrogen receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical staining for estrogen receptors in the endometrium was positive in all but one treated gilts , and negative to weakly positive in control gilts .
	manualset3
92859	3	399381	13	NULL	NULL	0	NULL	endometrium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical staining for estrogen receptors in the endometrium was positive in all but one treated gilts , and negative to weakly positive in control gilts .
	manualset3
92860	5	399381	13	NULL	NULL	NULL	NULL	gilts	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunohistochemical staining for estrogen receptors in the endometrium was positive in all but one treated gilts , and negative to weakly positive in control gilts .
	manualset3
92861	6	399381	13	NULL	NULL	NULL	NULL	control gilts	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunohistochemical staining for estrogen receptors in the endometrium was positive in all but one treated gilts , and negative to weakly positive in control gilts .
	manualset3
92862	4	399381	13	NULL	NULL	0	NULL	one 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical staining for estrogen receptors in the endometrium was positive in all but one treated gilts , and negative to weakly positive in control gilts .
	manualset3
92863	1	399382	13	NULL	NULL	0	NULL	Immunohistochemical staining	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical staining with a monoclonal antibody ( DO-7 ) and a polyclonal antibody ( CM-1 ) to p53 protein ( both wild type and mutant ) on formalin-fixed paraffin sections showed a strong correlation with malignancy grade .
	manualset3
92864	2	399382	13	NULL	NULL	0	NULL	monoclonal antibody ( DO-7 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical staining with a monoclonal antibody ( DO-7 ) and a polyclonal antibody ( CM-1 ) to p53 protein ( both wild type and mutant ) on formalin-fixed paraffin sections showed a strong correlation with malignancy grade .
	manualset3
92865	3	399382	13	NULL	NULL	0	NULL	polyclonal antibody ( CM-1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical staining with a monoclonal antibody ( DO-7 ) and a polyclonal antibody ( CM-1 ) to p53 protein ( both wild type and mutant ) on formalin-fixed paraffin sections showed a strong correlation with malignancy grade .
	manualset3
92866	4	399382	13	NULL	NULL	0	NULL	p53 protein ( both wild type and mutant )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical staining with a monoclonal antibody ( DO-7 ) and a polyclonal antibody ( CM-1 ) to p53 protein ( both wild type and mutant ) on formalin-fixed paraffin sections showed a strong correlation with malignancy grade .
	manualset3
92867	5	399382	13	NULL	NULL	NULL	NULL	formalin-fixed paraffin sections 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunohistochemical staining with a monoclonal antibody ( DO-7 ) and a polyclonal antibody ( CM-1 ) to p53 protein ( both wild type and mutant ) on formalin-fixed paraffin sections showed a strong correlation with malignancy grade .
	manualset3
92868	6	399382	13	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical staining with a monoclonal antibody ( DO-7 ) and a polyclonal antibody ( CM-1 ) to p53 protein ( both wild type and mutant ) on formalin-fixed paraffin sections showed a strong correlation with malignancy grade .
	manualset3
92869	7	399382	13	NULL	NULL	0	NULL	malignancy grade	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical staining with a monoclonal antibody ( DO-7 ) and a polyclonal antibody ( CM-1 ) to p53 protein ( both wild type and mutant ) on formalin-fixed paraffin sections showed a strong correlation with malignancy grade .
	manualset3
92870	1	399383	13	NULL	NULL	0	NULL	Immunohistochemical stains 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical stains for synaptophysin and chromogranin demonstrated diffuse , strong positivity uniformly throughout the tumor , even in the more conventional-appearing areas .
	manualset3
92871	2	399383	13	NULL	NULL	0	NULL	synaptophysin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical stains for synaptophysin and chromogranin demonstrated diffuse , strong positivity uniformly throughout the tumor , even in the more conventional-appearing areas .
	manualset3
92872	3	399383	13	NULL	NULL	0	NULL	chromogranin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical stains for synaptophysin and chromogranin demonstrated diffuse , strong positivity uniformly throughout the tumor , even in the more conventional-appearing areas .
	manualset3
92873	5	399383	13	NULL	NULL	NULL	NULL	tumor 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunohistochemical stains for synaptophysin and chromogranin demonstrated diffuse , strong positivity uniformly throughout the tumor , even in the more conventional-appearing areas .
	manualset3
92874	6	399383	13	NULL	NULL	NULL	NULL	conventional-appearing areas 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunohistochemical stains for synaptophysin and chromogranin demonstrated diffuse , strong positivity uniformly throughout the tumor , even in the more conventional-appearing areas .
	manualset3
92875	4	399383	13	NULL	NULL	0	NULL	positivity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical stains for synaptophysin and chromogranin demonstrated diffuse , strong positivity uniformly throughout the tumor , even in the more conventional-appearing areas .
	manualset3
92876	1	399384	13	NULL	NULL	0	NULL	Immunohistochemical study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical study on neuroglia identified by the monoclonal antibody against a macrophage differentiation antigen ( Mac-1 ) .
	manualset3
92877	2	399384	13	NULL	NULL	0	NULL	neuroglia	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical study on neuroglia identified by the monoclonal antibody against a macrophage differentiation antigen ( Mac-1 ) .
	manualset3
92878	3	399384	13	NULL	NULL	0	NULL	monoclonal antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical study on neuroglia identified by the monoclonal antibody against a macrophage differentiation antigen ( Mac-1 ) .
	manualset3
92879	4	399384	13	NULL	NULL	0	NULL	macrophage differentiation antigen ( Mac-1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical study on neuroglia identified by the monoclonal antibody against a macrophage differentiation antigen ( Mac-1 ) .
	manualset3
92881	2	399385	13	NULL	NULL	0	NULL	tumor cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemically , the tumor cells were labeled by antibodies against neurofilament protein , synaptophysin , glial fibrillary acidic protein and S-100 protein antigen , but were negative for chromogranin A , cytokeratin and desmin .
	manualset3
92882	3	399385	13	NULL	NULL	0	NULL	antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemically , the tumor cells were labeled by antibodies against neurofilament protein , synaptophysin , glial fibrillary acidic protein and S-100 protein antigen , but were negative for chromogranin A , cytokeratin and desmin .
	manualset3
92883	4	399385	13	NULL	NULL	0	NULL	neurofilament protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemically , the tumor cells were labeled by antibodies against neurofilament protein , synaptophysin , glial fibrillary acidic protein and S-100 protein antigen , but were negative for chromogranin A , cytokeratin and desmin .
	manualset3
92884	5	399385	13	NULL	NULL	0	NULL	synaptophysin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemically , the tumor cells were labeled by antibodies against neurofilament protein , synaptophysin , glial fibrillary acidic protein and S-100 protein antigen , but were negative for chromogranin A , cytokeratin and desmin .
	manualset3
92885	6	399385	13	NULL	NULL	0	NULL	glial fibrillary acidic protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemically , the tumor cells were labeled by antibodies against neurofilament protein , synaptophysin , glial fibrillary acidic protein and S-100 protein antigen , but were negative for chromogranin A , cytokeratin and desmin .
	manualset3
92886	7	399385	13	NULL	NULL	NULL	NULL	 S-100 protein antigen	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunohistochemically , the tumor cells were labeled by antibodies against neurofilament protein , synaptophysin , glial fibrillary acidic protein and S-100 protein antigen , but were negative for chromogranin A , cytokeratin and desmin .
	manualset3
92887	8	399385	13	NULL	NULL	0	NULL	 chromogranin A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemically , the tumor cells were labeled by antibodies against neurofilament protein , synaptophysin , glial fibrillary acidic protein and S-100 protein antigen , but were negative for chromogranin A , cytokeratin and desmin .
	manualset3
92888	9	399385	13	NULL	NULL	0	NULL	cytokeratin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemically , the tumor cells were labeled by antibodies against neurofilament protein , synaptophysin , glial fibrillary acidic protein and S-100 protein antigen , but were negative for chromogranin A , cytokeratin and desmin .
	manualset3
92889	10	399385	13	NULL	NULL	0	NULL	desmin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemically , the tumor cells were labeled by antibodies against neurofilament protein , synaptophysin , glial fibrillary acidic protein and S-100 protein antigen , but were negative for chromogranin A , cytokeratin and desmin .
	manualset3
92890	1	399386	13	NULL	NULL	0	NULL	Immunolabeling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunolabeling of SSPE and wild-type measles viruses in ferret brain cell culture .
	manualset3
92891	2	399386	13	NULL	NULL	0	NULL	SSPE	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunolabeling of SSPE and wild-type measles viruses in ferret brain cell culture .
	manualset3
92892	3	399386	13	NULL	NULL	0	NULL	wild-type measles viruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunolabeling of SSPE and wild-type measles viruses in ferret brain cell culture .
	manualset3
92893	4	399386	13	NULL	NULL	0	NULL	ferret brain cell culture 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunolabeling of SSPE and wild-type measles viruses in ferret brain cell culture .
	manualset3
92894	1	399387	13	NULL	NULL	0	NULL	Immunologic criteria	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunologic criteria are poor predictors of virologic outcome : implications for HIV treatment monitoring in resource-limited settings .
	manualset3
92895	2	399387	13	NULL	NULL	NULL	NULL	 predictors of virologic outcome	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunologic criteria are poor predictors of virologic outcome : implications for HIV treatment monitoring in resource-limited settings .
	manualset3
92896	3	399387	13	NULL	NULL	0	NULL	implications 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunologic criteria are poor predictors of virologic outcome : implications for HIV treatment monitoring in resource-limited settings .
	manualset3
92897	4	399387	13	NULL	NULL	0	NULL	HIV treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunologic criteria are poor predictors of virologic outcome : implications for HIV treatment monitoring in resource-limited settings .
	manualset3
92898	5	399387	13	NULL	NULL	0	NULL	resource-limited settings 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunologic criteria are poor predictors of virologic outcome : implications for HIV treatment monitoring in resource-limited settings .
	manualset3
92899	1	399388	13	NULL	NULL	0	NULL	Immunologic mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunologic mechanisms and aberrations of the RAS have been long considered contributors to the disorder .
	manualset3
92900	2	399388	13	NULL	NULL	0	NULL	aberrations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunologic mechanisms and aberrations of the RAS have been long considered contributors to the disorder .
	manualset3
92901	3	399388	13	NULL	NULL	0	NULL	RAS	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunologic mechanisms and aberrations of the RAS have been long considered contributors to the disorder .
	manualset3
92902	4	399388	13	NULL	NULL	0	NULL	contributors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunologic mechanisms and aberrations of the RAS have been long considered contributors to the disorder .
	manualset3
92903	5	399388	13	NULL	NULL	0	NULL	 disorder	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunologic mechanisms and aberrations of the RAS have been long considered contributors to the disorder .
	manualset3
92905	1	399389	13	NULL	NULL	0	NULL	Immunological-focused microarray gene expression analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunological-focused microarray gene expression analysis showed that only the CD72 gene was significantly downregulated in the 12-month RSV-treated mice compared to age-matched controls .
	manualset3
92906	2	399389	13	NULL	NULL	0	NULL	 CD72 gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunological-focused microarray gene expression analysis showed that only the CD72 gene was significantly downregulated in the 12-month RSV-treated mice compared to age-matched controls .
	manualset3
92907	3	399389	13	NULL	NULL	0	NULL	12-month RSV-treated mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunological-focused microarray gene expression analysis showed that only the CD72 gene was significantly downregulated in the 12-month RSV-treated mice compared to age-matched controls .
	manualset3
92908	4	399389	13	NULL	NULL	0	NULL	age-matched controls	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunological-focused microarray gene expression analysis showed that only the CD72 gene was significantly downregulated in the 12-month RSV-treated mice compared to age-matched controls .
	manualset3
92909	1	399390	13	NULL	NULL	0	NULL	Immunological aspects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunological aspects of transfer amyloidosis .
	manualset3
92910	2	399390	13	NULL	NULL	0	NULL	transfer amyloidosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunological aspects of transfer amyloidosis .
	manualset3
92911	1	399391	13	NULL	NULL	0	NULL	Immunological response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunological response related to photodynamic therapy ( PDT ) is one of the basic elements that influence on the efficiency of this cancer treatment method .
	manualset3
92912	2	399391	13	NULL	NULL	0	NULL	photodynamic therapy ( PDT )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunological response related to photodynamic therapy ( PDT ) is one of the basic elements that influence on the efficiency of this cancer treatment method .
	manualset3
92913	3	399391	13	NULL	NULL	0	NULL	basic elements	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunological response related to photodynamic therapy ( PDT ) is one of the basic elements that influence on the efficiency of this cancer treatment method .
	manualset3
92915	5	399391	13	NULL	NULL	NULL	NULL	efficiency	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunological response related to photodynamic therapy ( PDT ) is one of the basic elements that influence on the efficiency of this cancer treatment method .
	manualset3
92916	6	399391	13	NULL	NULL	NULL	NULL	cancer treatment method	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunological response related to photodynamic therapy ( PDT ) is one of the basic elements that influence on the efficiency of this cancer treatment method .
	manualset3
92917	1	399392	13	NULL	NULL	0	NULL	Immunological studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunological studies indicate that the Mr-24 , 500 subunits present in GST III ( pI 7.9 ) are distinct from those present in GST IV ( pI 6.4 ) and V ( pI 5.7 ) .
	manualset3
92918	2	399392	13	NULL	NULL	0	NULL	Mr-24 , 500 subunits	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunological studies indicate that the Mr-24 , 500 subunits present in GST III ( pI 7.9 ) are distinct from those present in GST IV ( pI 6.4 ) and V ( pI 5.7 ) .
	manualset3
92919	3	399392	13	NULL	NULL	0	NULL	GST III ( pI 7.9 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunological studies indicate that the Mr-24 , 500 subunits present in GST III ( pI 7.9 ) are distinct from those present in GST IV ( pI 6.4 ) and V ( pI 5.7 ) .
	manualset3
92920	4	399392	13	NULL	NULL	0	NULL	GST IV ( pI 6.4 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunological studies indicate that the Mr-24 , 500 subunits present in GST III ( pI 7.9 ) are distinct from those present in GST IV ( pI 6.4 ) and V ( pI 5.7 ) .
	manualset3
92922	5	399392	13	NULL	NULL	0	NULL	GST V ( pI 5.7 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunological studies indicate that the Mr-24 , 500 subunits present in GST III ( pI 7.9 ) are distinct from those present in GST IV ( pI 6.4 ) and V ( pI 5.7 ) .
	manualset3
92923	1	399393	13	NULL	NULL	0	NULL	Immunological variations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunological variations of albumin as a function of the degradation stage ) .
	manualset3
92924	2	399393	13	NULL	NULL	0	NULL	albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunological variations of albumin as a function of the degradation stage ) .
	manualset3
92925	3	399393	13	NULL	NULL	NULL	NULL	function of the degradation stage	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunological variations of albumin as a function of the degradation stage ) .
	manualset3
92926	1	399394	13	NULL	NULL	NULL	NULL	food allergy	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunologically mediated food allergy : the importance of food challenge procedures .
	manualset3
92927	2	399394	13	NULL	NULL	0	NULL	importance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunologically mediated food allergy : the importance of food challenge procedures .
	manualset3
92928	3	399394	13	NULL	NULL	0	NULL	food challenge procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunologically mediated food allergy : the importance of food challenge procedures .
	manualset3
92929	1	399395	13	NULL	NULL	0	NULL	Immunoperoxidase studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoperoxidase studies using antibodies LN1 , LN2 , and L26 confirmed the presence of B cells in thymomas , particularly those with germinal centers .
	manualset3
92930	2	399395	13	NULL	NULL	0	NULL	antibodies LN1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoperoxidase studies using antibodies LN1 , LN2 , and L26 confirmed the presence of B cells in thymomas , particularly those with germinal centers .
	manualset3
92931	3	399395	13	NULL	NULL	0	NULL	antibodies LN2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoperoxidase studies using antibodies LN1 , LN2 , and L26 confirmed the presence of B cells in thymomas , particularly those with germinal centers .
	manualset3
92932	4	399395	13	NULL	NULL	0	NULL	antibodies L26	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoperoxidase studies using antibodies LN1 , LN2 , and L26 confirmed the presence of B cells in thymomas , particularly those with germinal centers .
	manualset3
92933	6	399395	13	NULL	NULL	NULL	NULL	B cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunoperoxidase studies using antibodies LN1 , LN2 , and L26 confirmed the presence of B cells in thymomas , particularly those with germinal centers .
	manualset3
92934	7	399395	13	NULL	NULL	NULL	NULL	thymomas	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunoperoxidase studies using antibodies LN1 , LN2 , and L26 confirmed the presence of B cells in thymomas , particularly those with germinal centers .
	manualset3
92935	8	399395	13	NULL	NULL	NULL	NULL	germinal centers	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunoperoxidase studies using antibodies LN1 , LN2 , and L26 confirmed the presence of B cells in thymomas , particularly those with germinal centers .
	manualset3
92936	5	399395	13	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoperoxidase studies using antibodies LN1 , LN2 , and L26 confirmed the presence of B cells in thymomas , particularly those with germinal centers .
	manualset3
92937	1	399396	13	NULL	NULL	0	NULL	Immunopositivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunopositivity was detected in the tumors tested as follows : KIT , 100 % ; CD34 , 75 % ; PKCtheta , 21 % ; PDGFRA , 90 % ; and smooth muscle actin , 6 % .
	manualset3
92938	2	399396	13	NULL	NULL	0	NULL	tumors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunopositivity was detected in the tumors tested as follows : KIT , 100 % ; CD34 , 75 % ; PKCtheta , 21 % ; PDGFRA , 90 % ; and smooth muscle actin , 6 % .
	manualset3
92939	3	399396	13	NULL	NULL	0	NULL	KIT	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunopositivity was detected in the tumors tested as follows : KIT , 100 % ; CD34 , 75 % ; PKCtheta , 21 % ; PDGFRA , 90 % ; and smooth muscle actin , 6 % .
	manualset3
92940	4	399396	13	NULL	NULL	0	NULL	100 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunopositivity was detected in the tumors tested as follows : KIT , 100 % ; CD34 , 75 % ; PKCtheta , 21 % ; PDGFRA , 90 % ; and smooth muscle actin , 6 % .
	manualset3
92941	5	399396	13	NULL	NULL	0	NULL	CD34	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunopositivity was detected in the tumors tested as follows : KIT , 100 % ; CD34 , 75 % ; PKCtheta , 21 % ; PDGFRA , 90 % ; and smooth muscle actin , 6 % .
	manualset3
92942	6	399396	13	NULL	NULL	0	NULL	75 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunopositivity was detected in the tumors tested as follows : KIT , 100 % ; CD34 , 75 % ; PKCtheta , 21 % ; PDGFRA , 90 % ; and smooth muscle actin , 6 % .
	manualset3
92943	7	399396	13	NULL	NULL	0	NULL	PKCtheta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunopositivity was detected in the tumors tested as follows : KIT , 100 % ; CD34 , 75 % ; PKCtheta , 21 % ; PDGFRA , 90 % ; and smooth muscle actin , 6 % .
	manualset3
92944	8	399396	13	NULL	NULL	0	NULL	 21 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunopositivity was detected in the tumors tested as follows : KIT , 100 % ; CD34 , 75 % ; PKCtheta , 21 % ; PDGFRA , 90 % ; and smooth muscle actin , 6 % .
	manualset3
92945	9	399396	13	NULL	NULL	0	NULL	 PDGFRA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunopositivity was detected in the tumors tested as follows : KIT , 100 % ; CD34 , 75 % ; PKCtheta , 21 % ; PDGFRA , 90 % ; and smooth muscle actin , 6 % .
	manualset3
92946	10	399396	13	NULL	NULL	0	NULL	90 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunopositivity was detected in the tumors tested as follows : KIT , 100 % ; CD34 , 75 % ; PKCtheta , 21 % ; PDGFRA , 90 % ; and smooth muscle actin , 6 % .
	manualset3
92947	11	399396	13	NULL	NULL	0	NULL	smooth muscle actin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunopositivity was detected in the tumors tested as follows : KIT , 100 % ; CD34 , 75 % ; PKCtheta , 21 % ; PDGFRA , 90 % ; and smooth muscle actin , 6 % .
	manualset3
92948	12	399396	13	NULL	NULL	0	NULL	 6 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunopositivity was detected in the tumors tested as follows : KIT , 100 % ; CD34 , 75 % ; PKCtheta , 21 % ; PDGFRA , 90 % ; and smooth muscle actin , 6 % .
	manualset3
92949	1	399397	13	NULL	NULL	0	NULL	Immunoprecipitation analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation analyses of B-CLL sera allow detection of several high molecular weight bands and of a 78 kDa band that represents a soluble form of CD44st and is 4 kDa lower than a similar band ( 82 kDa ) detected in B-CLL cell lysates .
	manualset3
92950	2	399397	13	NULL	NULL	0	NULL	B-CLL sera	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation analyses of B-CLL sera allow detection of several high molecular weight bands and of a 78 kDa band that represents a soluble form of CD44st and is 4 kDa lower than a similar band ( 82 kDa ) detected in B-CLL cell lysates .
	manualset3
92951	3	399397	13	NULL	NULL	0	NULL	detection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation analyses of B-CLL sera allow detection of several high molecular weight bands and of a 78 kDa band that represents a soluble form of CD44st and is 4 kDa lower than a similar band ( 82 kDa ) detected in B-CLL cell lysates .
	manualset3
92953	4	399397	13	NULL	NULL	0	NULL	several high molecular weight bands	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation analyses of B-CLL sera allow detection of several high molecular weight bands and of a 78 kDa band that represents a soluble form of CD44st and is 4 kDa lower than a similar band ( 82 kDa ) detected in B-CLL cell lysates .
	manualset3
92954	5	399397	13	NULL	NULL	NULL	NULL	78 kDa band	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation analyses of B-CLL sera allow detection of several high molecular weight bands and of a 78 kDa band that represents a soluble form of CD44st and is 4 kDa lower than a similar band ( 82 kDa ) detected in B-CLL cell lysates .
	manualset3
92955	6	399397	13	NULL	NULL	0	NULL	soluble form of CD44st	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation analyses of B-CLL sera allow detection of several high molecular weight bands and of a 78 kDa band that represents a soluble form of CD44st and is 4 kDa lower than a similar band ( 82 kDa ) detected in B-CLL cell lysates .
	manualset3
92956	7	399397	13	NULL	NULL	0	NULL	 4 kDa lower than a similar band ( 82 kDa ) 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation analyses of B-CLL sera allow detection of several high molecular weight bands and of a 78 kDa band that represents a soluble form of CD44st and is 4 kDa lower than a similar band ( 82 kDa ) detected in B-CLL cell lysates .
	manualset3
92958	8	399397	13	NULL	NULL	0	NULL	B-CLL cell lysates	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation analyses of B-CLL sera allow detection of several high molecular weight bands and of a 78 kDa band that represents a soluble form of CD44st and is 4 kDa lower than a similar band ( 82 kDa ) detected in B-CLL cell lysates .
	manualset3
92963	1	399398	13	NULL	NULL	0	NULL	Immunoprecipitation analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation analysis of radiolabeled conditioned medium revealed a specific Mr 25 , 000 band only after acidification .
	manualset3
92964	2	399398	13	NULL	NULL	NULL	NULL	conditioned medium	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation analysis of radiolabeled conditioned medium revealed a specific Mr 25 , 000 band only after acidification .
	manualset3
92965	3	399398	13	NULL	NULL	0	NULL	Mr 25 , 000 band	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation analysis of radiolabeled conditioned medium revealed a specific Mr 25 , 000 band only after acidification .
	manualset3
92966	4	399398	13	NULL	NULL	0	NULL	acidification 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation analysis of radiolabeled conditioned medium revealed a specific Mr 25 , 000 band only after acidification .
	manualset3
92976	1	399399	13	NULL	NULL	0	NULL	Immunoprecipitation experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation experiments using peptide-specific anti-SBE antibodies showed that SBEIIb and starch phosphorylase each coimmunoprecipitated with SBEI in a phosphorylation-dependent manner , suggesting that these enzymes may form protein complexes within the amyloplast in vivo .
	manualset3
92977	2	399399	13	NULL	NULL	0	NULL	peptide-specific anti-SBE antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation experiments using peptide-specific anti-SBE antibodies showed that SBEIIb and starch phosphorylase each coimmunoprecipitated with SBEI in a phosphorylation-dependent manner , suggesting that these enzymes may form protein complexes within the amyloplast in vivo .
	manualset3
92978	3	399399	13	NULL	NULL	0	NULL	SBEIIb 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation experiments using peptide-specific anti-SBE antibodies showed that SBEIIb and starch phosphorylase each coimmunoprecipitated with SBEI in a phosphorylation-dependent manner , suggesting that these enzymes may form protein complexes within the amyloplast in vivo .
	manualset3
92979	4	399399	13	NULL	NULL	0	NULL	starch phosphorylase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation experiments using peptide-specific anti-SBE antibodies showed that SBEIIb and starch phosphorylase each coimmunoprecipitated with SBEI in a phosphorylation-dependent manner , suggesting that these enzymes may form protein complexes within the amyloplast in vivo .
	manualset3
92980	5	399399	13	NULL	NULL	0	NULL	SBEI	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation experiments using peptide-specific anti-SBE antibodies showed that SBEIIb and starch phosphorylase each coimmunoprecipitated with SBEI in a phosphorylation-dependent manner , suggesting that these enzymes may form protein complexes within the amyloplast in vivo .
	manualset3
92981	6	399399	13	NULL	NULL	0	NULL	 phosphorylation-dependent manner	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation experiments using peptide-specific anti-SBE antibodies showed that SBEIIb and starch phosphorylase each coimmunoprecipitated with SBEI in a phosphorylation-dependent manner , suggesting that these enzymes may form protein complexes within the amyloplast in vivo .
	manualset3
92982	7	399399	13	NULL	NULL	0	NULL	enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation experiments using peptide-specific anti-SBE antibodies showed that SBEIIb and starch phosphorylase each coimmunoprecipitated with SBEI in a phosphorylation-dependent manner , suggesting that these enzymes may form protein complexes within the amyloplast in vivo .
	manualset3
92983	8	399399	13	NULL	NULL	0	NULL	protein complexes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation experiments using peptide-specific anti-SBE antibodies showed that SBEIIb and starch phosphorylase each coimmunoprecipitated with SBEI in a phosphorylation-dependent manner , suggesting that these enzymes may form protein complexes within the amyloplast in vivo .
	manualset3
92984	9	399399	13	NULL	NULL	0	NULL	amyloplast	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation experiments using peptide-specific anti-SBE antibodies showed that SBEIIb and starch phosphorylase each coimmunoprecipitated with SBEI in a phosphorylation-dependent manner , suggesting that these enzymes may form protein complexes within the amyloplast in vivo .
	manualset3
92985	1	399400	13	NULL	NULL	0	NULL	Immunoprecipitation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation of MS2-tagged NCL 3 ` UTR was used to screen for endogenous repressors of nucleolin synthesis .
	manualset3
92986	2	399400	13	NULL	NULL	0	NULL	MS2-tagged NCL 3 ` UTR	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation of MS2-tagged NCL 3 ` UTR was used to screen for endogenous repressors of nucleolin synthesis .
	manualset3
92987	3	399400	13	NULL	NULL	0	NULL	endogenous repressors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation of MS2-tagged NCL 3 ` UTR was used to screen for endogenous repressors of nucleolin synthesis .
	manualset3
92988	4	399400	13	NULL	NULL	0	NULL	nucleolin synthesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation of MS2-tagged NCL 3 ` UTR was used to screen for endogenous repressors of nucleolin synthesis .
	manualset3
92989	1	399401	13	NULL	NULL	0	NULL	Immunoprecipitation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation of their livers followed by autoradiographic analysis showed the presence of 32P in small molecular weight apo-B .
	manualset3
92990	2	399401	13	NULL	NULL	0	NULL	livers 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation of their livers followed by autoradiographic analysis showed the presence of 32P in small molecular weight apo-B .
	manualset3
92991	3	399401	13	NULL	NULL	0	NULL	autoradiographic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation of their livers followed by autoradiographic analysis showed the presence of 32P in small molecular weight apo-B .
	manualset3
92992	4	399401	13	NULL	NULL	0	NULL	32P	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation of their livers followed by autoradiographic analysis showed the presence of 32P in small molecular weight apo-B .
	manualset3
92993	5	399401	13	NULL	NULL	0	NULL	small molecular weight apo-B 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation of their livers followed by autoradiographic analysis showed the presence of 32P in small molecular weight apo-B .
	manualset3
92994	1	399402	13	NULL	NULL	0	NULL	Immunoprofile	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprofile of Hodgkin 's lymphoma in India .
	manualset3
92995	2	399402	13	NULL	NULL	0	NULL	Hodgkin 's lymphoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprofile of Hodgkin 's lymphoma in India .
	manualset3
92996	3	399402	13	NULL	NULL	0	NULL	India 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprofile of Hodgkin 's lymphoma in India .
	manualset3
92997	1	399403	13	NULL	NULL	0	NULL	Immunoprophylaxis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprophylaxis with Simulect ( basiliximab ) in pediatric kidney transplant recipients : results from routine clinical practice at 5 kidney transplant units .
	manualset3
92998	2	399403	13	NULL	NULL	0	NULL	Simulect ( basiliximab ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprophylaxis with Simulect ( basiliximab ) in pediatric kidney transplant recipients : results from routine clinical practice at 5 kidney transplant units .
	manualset3
92999	3	399403	13	NULL	NULL	0	NULL	pediatric kidney transplant recipients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprophylaxis with Simulect ( basiliximab ) in pediatric kidney transplant recipients : results from routine clinical practice at 5 kidney transplant units .
	manualset3
93000	5	399403	13	NULL	NULL	NULL	NULL	routine clinical practice	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunoprophylaxis with Simulect ( basiliximab ) in pediatric kidney transplant recipients : results from routine clinical practice at 5 kidney transplant units .
	manualset3
93001	6	399403	13	NULL	NULL	NULL	NULL	5 kidney transplant units	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunoprophylaxis with Simulect ( basiliximab ) in pediatric kidney transplant recipients : results from routine clinical practice at 5 kidney transplant units .
	manualset3
93002	4	399403	13	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunoprophylaxis with Simulect ( basiliximab ) in pediatric kidney transplant recipients : results from routine clinical practice at 5 kidney transplant units .
	manualset3
93020	1	399404	13	NULL	NULL	0	NULL	Immunoreactive ( i ) TxB2 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoreactive ( i ) TxB2 was measured in plasma or Fluosol-43 obtained from rats prior to and after injection of Salmonella enteritidis endotoxin ( 20 mg/kg ) .
	manualset3
93021	2	399404	13	NULL	NULL	0	NULL	 plasma 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoreactive ( i ) TxB2 was measured in plasma or Fluosol-43 obtained from rats prior to and after injection of Salmonella enteritidis endotoxin ( 20 mg/kg ) .
	manualset3
93022	3	399404	13	NULL	NULL	0	NULL	Fluosol-43	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoreactive ( i ) TxB2 was measured in plasma or Fluosol-43 obtained from rats prior to and after injection of Salmonella enteritidis endotoxin ( 20 mg/kg ) .
	manualset3
93023	4	399404	13	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoreactive ( i ) TxB2 was measured in plasma or Fluosol-43 obtained from rats prior to and after injection of Salmonella enteritidis endotoxin ( 20 mg/kg ) .
	manualset3
93024	5	399404	13	NULL	NULL	0	NULL	injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoreactive ( i ) TxB2 was measured in plasma or Fluosol-43 obtained from rats prior to and after injection of Salmonella enteritidis endotoxin ( 20 mg/kg ) .
	manualset3
93025	6	399404	13	NULL	NULL	0	NULL	Salmonella enteritidis endotoxin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoreactive ( i ) TxB2 was measured in plasma or Fluosol-43 obtained from rats prior to and after injection of Salmonella enteritidis endotoxin ( 20 mg/kg ) .
	manualset3
93026	7	399404	13	NULL	NULL	0	NULL	20 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoreactive ( i ) TxB2 was measured in plasma or Fluosol-43 obtained from rats prior to and after injection of Salmonella enteritidis endotoxin ( 20 mg/kg ) .
	manualset3
93027	1	399405	13	NULL	NULL	0	NULL	Therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Therapy of intestinal infections with paromomycin ) .
	manualset3
93028	2	399405	13	NULL	NULL	0	NULL	intestinal infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Therapy of intestinal infections with paromomycin ) .
	manualset3
93029	3	399405	13	NULL	NULL	0	NULL	paromomycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Therapy of intestinal infections with paromomycin ) .
	manualset3
93030	1	399406	13	NULL	NULL	0	NULL	Immunoreactive bradykinin ( IRBK )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoreactive bradykinin ( IRBK ) was measured in the perfusate and the basal level was found to be constant for up to 3 h. Ten min perfusions of the hearts with ET-1 at concentrations of 0.2-20 pM produced a dose-related suppression of kinin outflow by over 90 % ( P & lt ; 0.05 ) .
	manualset3
93031	2	399406	13	NULL	NULL	0	NULL	perfusate level  	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoreactive bradykinin ( IRBK ) was measured in the perfusate and the basal level was found to be constant for up to 3 h. Ten min perfusions of the hearts with ET-1 at concentrations of 0.2-20 pM produced a dose-related suppression of kinin outflow by over 90 % ( P & lt ; 0.05 ) .
	manualset3
93032	3	399406	13	NULL	NULL	0	NULL	basal level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoreactive bradykinin ( IRBK ) was measured in the perfusate and the basal level was found to be constant for up to 3 h. Ten min perfusions of the hearts with ET-1 at concentrations of 0.2-20 pM produced a dose-related suppression of kinin outflow by over 90 % ( P & lt ; 0.05 ) .
	manualset3
93033	4	399406	13	NULL	NULL	0	NULL	3 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoreactive bradykinin ( IRBK ) was measured in the perfusate and the basal level was found to be constant for up to 3 h. Ten min perfusions of the hearts with ET-1 at concentrations of 0.2-20 pM produced a dose-related suppression of kinin outflow by over 90 % ( P & lt ; 0.05 ) .
	manualset3
93034	5	399406	13	NULL	NULL	0	NULL	Ten min	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoreactive bradykinin ( IRBK ) was measured in the perfusate and the basal level was found to be constant for up to 3 h. Ten min perfusions of the hearts with ET-1 at concentrations of 0.2-20 pM produced a dose-related suppression of kinin outflow by over 90 % ( P & lt ; 0.05 ) .
	manualset3
93035	6	399406	13	NULL	NULL	0	NULL	perfusions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoreactive bradykinin ( IRBK ) was measured in the perfusate and the basal level was found to be constant for up to 3 h. Ten min perfusions of the hearts with ET-1 at concentrations of 0.2-20 pM produced a dose-related suppression of kinin outflow by over 90 % ( P & lt ; 0.05 ) .
	manualset3
93036	7	399406	13	NULL	NULL	0	NULL	 hearts 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoreactive bradykinin ( IRBK ) was measured in the perfusate and the basal level was found to be constant for up to 3 h. Ten min perfusions of the hearts with ET-1 at concentrations of 0.2-20 pM produced a dose-related suppression of kinin outflow by over 90 % ( P & lt ; 0.05 ) .
	manualset3
93037	8	399406	13	NULL	NULL	NULL	NULL	ET-1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunoreactive bradykinin ( IRBK ) was measured in the perfusate and the basal level was found to be constant for up to 3 h. Ten min perfusions of the hearts with ET-1 at concentrations of 0.2-20 pM produced a dose-related suppression of kinin outflow by over 90 % ( P & lt ; 0.05 ) .
	manualset3
93038	9	399406	13	NULL	NULL	0	NULL	concentrations of 0.2-20 pM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoreactive bradykinin ( IRBK ) was measured in the perfusate and the basal level was found to be constant for up to 3 h. Ten min perfusions of the hearts with ET-1 at concentrations of 0.2-20 pM produced a dose-related suppression of kinin outflow by over 90 % ( P & lt ; 0.05 ) .
	manualset3
93039	10	399406	13	NULL	NULL	NULL	NULL	dose-related suppression of kinin outflow  	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunoreactive bradykinin ( IRBK ) was measured in the perfusate and the basal level was found to be constant for up to 3 h. Ten min perfusions of the hearts with ET-1 at concentrations of 0.2-20 pM produced a dose-related suppression of kinin outflow by over 90 % ( P & lt ; 0.05 ) .
	manualset3
93040	11	399406	13	NULL	NULL	0	NULL	over 90 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoreactive bradykinin ( IRBK ) was measured in the perfusate and the basal level was found to be constant for up to 3 h. Ten min perfusions of the hearts with ET-1 at concentrations of 0.2-20 pM produced a dose-related suppression of kinin outflow by over 90 % ( P & lt ; 0.05 ) .
	manualset3
93041	12	399406	13	NULL	NULL	0	NULL	P & lt ; 0.05 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoreactive bradykinin ( IRBK ) was measured in the perfusate and the basal level was found to be constant for up to 3 h. Ten min perfusions of the hearts with ET-1 at concentrations of 0.2-20 pM produced a dose-related suppression of kinin outflow by over 90 % ( P & lt ; 0.05 ) .
	manualset3
93042	1	399407	13	NULL	NULL	0	NULL	Immunoreactive cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoreactive cells were found in about 2/3 of the tumors .
	manualset3
93043	2	399407	13	NULL	NULL	0	NULL	2/3 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoreactive cells were found in about 2/3 of the tumors .
	manualset3
93044	3	399407	13	NULL	NULL	0	NULL	 tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoreactive cells were found in about 2/3 of the tumors .
	manualset3
93045	1	399408	13	NULL	NULL	0	NULL	Immunosenescence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunosenescence is characterized by reduced levels of the peripheral naive T cell pool derived from thymus and the loss of immature B lineage cells in the bone marrow .
	manualset3
93046	2	399408	13	NULL	NULL	NULL	NULL	reduced levels	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunosenescence is characterized by reduced levels of the peripheral naive T cell pool derived from thymus and the loss of immature B lineage cells in the bone marrow .
	manualset3
93047	3	399408	13	NULL	NULL	0	NULL	peripheral naive T cell pool	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunosenescence is characterized by reduced levels of the peripheral naive T cell pool derived from thymus and the loss of immature B lineage cells in the bone marrow .
	manualset3
93048	4	399408	13	NULL	NULL	0	NULL	thymus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunosenescence is characterized by reduced levels of the peripheral naive T cell pool derived from thymus and the loss of immature B lineage cells in the bone marrow .
	manualset3
93049	5	399408	13	NULL	NULL	0	NULL	loss 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunosenescence is characterized by reduced levels of the peripheral naive T cell pool derived from thymus and the loss of immature B lineage cells in the bone marrow .
	manualset3
93050	6	399408	13	NULL	NULL	0	NULL	immature B lineage cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunosenescence is characterized by reduced levels of the peripheral naive T cell pool derived from thymus and the loss of immature B lineage cells in the bone marrow .
	manualset3
93051	7	399408	13	NULL	NULL	0	NULL	bone marrow	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunosenescence is characterized by reduced levels of the peripheral naive T cell pool derived from thymus and the loss of immature B lineage cells in the bone marrow .
	manualset3
93052	1	399409	13	NULL	NULL	0	NULL	Immunostaining	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunostaining and protein tagging demonstrated that only Dmc1p formed strong DSB-dependent foci on meiotic chromatin , whereas the distribution of Rad51p was diffuse within nuclei .
	manualset3
93053	2	399409	13	NULL	NULL	0	NULL	 protein tagging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunostaining and protein tagging demonstrated that only Dmc1p formed strong DSB-dependent foci on meiotic chromatin , whereas the distribution of Rad51p was diffuse within nuclei .
	manualset3
93054	3	399409	13	NULL	NULL	0	NULL	Dmc1p	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunostaining and protein tagging demonstrated that only Dmc1p formed strong DSB-dependent foci on meiotic chromatin , whereas the distribution of Rad51p was diffuse within nuclei .
	manualset3
93055	4	399409	13	NULL	NULL	0	NULL	DSB-dependent foci on meiotic chromatin	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunostaining and protein tagging demonstrated that only Dmc1p formed strong DSB-dependent foci on meiotic chromatin , whereas the distribution of Rad51p was diffuse within nuclei .
	manualset3
93056	5	399409	13	NULL	NULL	0	NULL	distribution 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunostaining and protein tagging demonstrated that only Dmc1p formed strong DSB-dependent foci on meiotic chromatin , whereas the distribution of Rad51p was diffuse within nuclei .
	manualset3
93057	6	399409	13	NULL	NULL	0	NULL	Rad51p	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunostaining and protein tagging demonstrated that only Dmc1p formed strong DSB-dependent foci on meiotic chromatin , whereas the distribution of Rad51p was diffuse within nuclei .
	manualset3
93059	7	399409	13	NULL	NULL	NULL	NULL	nuclei 	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Immunostaining and protein tagging demonstrated that only Dmc1p formed strong DSB-dependent foci on meiotic chromatin , whereas the distribution of Rad51p was diffuse within nuclei .
	manualset3
93060	1	399410	13	NULL	NULL	0	NULL	Immunostaining 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunostaining with HIK1083 and anti-lysozyme antibody was examined under light and electron microscopes .
	manualset3
93061	2	399410	13	NULL	NULL	0	NULL	HIK1083	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunostaining with HIK1083 and anti-lysozyme antibody was examined under light and electron microscopes .
	manualset3
93062	3	399410	13	NULL	NULL	0	NULL	anti-lysozyme antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunostaining with HIK1083 and anti-lysozyme antibody was examined under light and electron microscopes .
	manualset3
93063	4	399410	13	NULL	NULL	0	NULL	 light microscopes	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunostaining with HIK1083 and anti-lysozyme antibody was examined under light and electron microscopes .
	manualset3
93064	5	399410	13	NULL	NULL	0	NULL	electron microscopes	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunostaining with HIK1083 and anti-lysozyme antibody was examined under light and electron microscopes .
	manualset3
93065	1	399411	13	NULL	NULL	0	NULL	Immunotoxic effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunotoxic effects of diethylstilbestrol ( DES ) and cadmium chloride ( CAD ) on host resistance : comparison with cyclophosphamide ( CPS ) .
	manualset3
93066	2	399411	13	NULL	NULL	0	NULL	diethylstilbestrol ( DES ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunotoxic effects of diethylstilbestrol ( DES ) and cadmium chloride ( CAD ) on host resistance : comparison with cyclophosphamide ( CPS ) .
	manualset3
93067	3	399411	13	NULL	NULL	0	NULL	cadmium chloride ( CAD )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunotoxic effects of diethylstilbestrol ( DES ) and cadmium chloride ( CAD ) on host resistance : comparison with cyclophosphamide ( CPS ) .
	manualset3
93068	4	399411	13	NULL	NULL	0	NULL	host resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunotoxic effects of diethylstilbestrol ( DES ) and cadmium chloride ( CAD ) on host resistance : comparison with cyclophosphamide ( CPS ) .
	manualset3
93069	5	399411	13	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunotoxic effects of diethylstilbestrol ( DES ) and cadmium chloride ( CAD ) on host resistance : comparison with cyclophosphamide ( CPS ) .
	manualset3
93070	6	399411	13	NULL	NULL	0	NULL	 cyclophosphamide ( CPS )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunotoxic effects of diethylstilbestrol ( DES ) and cadmium chloride ( CAD ) on host resistance : comparison with cyclophosphamide ( CPS ) .
	manualset3
93071	1	399412	13	NULL	NULL	0	NULL	 Impact 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of DOTS compared with DOTS-plus on multidrug resistant tuberculosis and tuberculosis deaths : decision analysis .
	manualset3
93072	2	399412	13	NULL	NULL	0	NULL	DOTS	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of DOTS compared with DOTS-plus on multidrug resistant tuberculosis and tuberculosis deaths : decision analysis .
	manualset3
93073	3	399412	13	NULL	NULL	0	NULL	DOTS-plus	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of DOTS compared with DOTS-plus on multidrug resistant tuberculosis and tuberculosis deaths : decision analysis .
	manualset3
93074	4	399412	13	NULL	NULL	0	NULL	multidrug resistant tuberculosis deaths 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of DOTS compared with DOTS-plus on multidrug resistant tuberculosis and tuberculosis deaths : decision analysis .
	manualset3
93075	5	399412	13	NULL	NULL	0	NULL	 tuberculosis deaths	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of DOTS compared with DOTS-plus on multidrug resistant tuberculosis and tuberculosis deaths : decision analysis .
	manualset3
93076	6	399412	13	NULL	NULL	0	NULL	decision analysis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of DOTS compared with DOTS-plus on multidrug resistant tuberculosis and tuberculosis deaths : decision analysis .
	manualset3
93078	3	399413	13	NULL	NULL	NULL	NULL	anorexia nervosa	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Impact of broadening definitions of anorexia nervosa on sample characteristics .
	manualset3
93079	4	399413	13	NULL	NULL	NULL	NULL	sample characteristics 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Impact of broadening definitions of anorexia nervosa on sample characteristics .
	manualset3
93080	2	399413	13	NULL	NULL	0	NULL	broadening definitions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of broadening definitions of anorexia nervosa on sample characteristics .
	manualset3
93090	1	399413	13	NULL	NULL	0	NULL	Impact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of broadening definitions of anorexia nervosa on sample characteristics .
	manualset3
93081	1	399414	13	NULL	NULL	NULL	NULL	Impact of changes	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Impact of changes in catheter management on infectious complications among children with central venous catheters .
	manualset3
93082	2	399414	13	NULL	NULL	0	NULL	catheter management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of changes in catheter management on infectious complications among children with central venous catheters .
	manualset3
93083	3	399414	13	NULL	NULL	0	NULL	infectious complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of changes in catheter management on infectious complications among children with central venous catheters .
	manualset3
93084	4	399414	13	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of changes in catheter management on infectious complications among children with central venous catheters .
	manualset3
93085	5	399414	13	NULL	NULL	0	NULL	central venous catheters 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of changes in catheter management on infectious complications among children with central venous catheters .
	manualset3
93086	2	399415	13	NULL	NULL	NULL	NULL	chronic kidney disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Impact of chronic kidney disease on carotid plaque vulnerability .
	manualset3
93087	2	399415	13	NULL	NULL	0	NULL	carotid plaque vulnerability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of chronic kidney disease on carotid plaque vulnerability .
	manualset3
93088	1	399415	13	NULL	NULL	NULL	NULL	Impact	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Impact of chronic kidney disease on carotid plaque vulnerability .
	manualset3
93091	1	399416	13	NULL	NULL	NULL	NULL	Impact	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Impact of congenital color vision deficiency on education and unintentional injuries : findings from the 1958 British birth cohort .
	manualset3
93092	2	399416	13	NULL	NULL	0	NULL	congenital color vision deficiency 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of congenital color vision deficiency on education and unintentional injuries : findings from the 1958 British birth cohort .
	manualset3
93093	3	399416	13	NULL	NULL	0	NULL	education	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of congenital color vision deficiency on education and unintentional injuries : findings from the 1958 British birth cohort .
	manualset3
93094	4	399416	13	NULL	NULL	0	NULL	unintentional injuries	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of congenital color vision deficiency on education and unintentional injuries : findings from the 1958 British birth cohort .
	manualset3
93095	5	399416	13	NULL	NULL	0	NULL	findings	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of congenital color vision deficiency on education and unintentional injuries : findings from the 1958 British birth cohort .
	manualset3
93096	6	399416	13	NULL	NULL	0	NULL	1958	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of congenital color vision deficiency on education and unintentional injuries : findings from the 1958 British birth cohort .
	manualset3
93097	7	399416	13	NULL	NULL	0	NULL	British birth cohort 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of congenital color vision deficiency on education and unintentional injuries : findings from the 1958 British birth cohort .
	manualset3
93098	1	399417	13	NULL	NULL	NULL	NULL	Impact	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Impact of depressive symptoms on visceral sensitivity among patients with different subtypes of irritable bowel syndrome .
	manualset3
93099	2	399417	13	NULL	NULL	0	NULL	depressive symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of depressive symptoms on visceral sensitivity among patients with different subtypes of irritable bowel syndrome .
	manualset3
93100	3	399417	13	NULL	NULL	0	NULL	visceral sensitivity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of depressive symptoms on visceral sensitivity among patients with different subtypes of irritable bowel syndrome .
	manualset3
93101	4	399417	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of depressive symptoms on visceral sensitivity among patients with different subtypes of irritable bowel syndrome .
	manualset3
93102	5	399417	13	NULL	NULL	0	NULL	different subtypes of irritable bowel syndrome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of depressive symptoms on visceral sensitivity among patients with different subtypes of irritable bowel syndrome .
	manualset3
93103	1	399418	13	NULL	NULL	0	NULL	Impact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of different case definitions for acute otitis media on the efficacy estimates of a pneumococcal conjugate vaccine .
	manualset3
93104	2	399418	13	NULL	NULL	NULL	NULL	different case definitions 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Impact of different case definitions for acute otitis media on the efficacy estimates of a pneumococcal conjugate vaccine .
	manualset3
93105	3	399418	13	NULL	NULL	0	NULL	acute otitis media	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of different case definitions for acute otitis media on the efficacy estimates of a pneumococcal conjugate vaccine .
	manualset3
93106	4	399418	13	NULL	NULL	0	NULL	efficacy estimates 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of different case definitions for acute otitis media on the efficacy estimates of a pneumococcal conjugate vaccine .
	manualset3
93107	5	399418	13	NULL	NULL	0	NULL	pneumococcal conjugate vaccine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of different case definitions for acute otitis media on the efficacy estimates of a pneumococcal conjugate vaccine .
	manualset3
93108	1	399419	13	NULL	NULL	0	NULL	Impact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of global transcriptional regulation by ArcA , ArcB , Cra , Crp , Cya , Fnr , and Mlc on glucose catabolism in Escherichia coli .
	manualset3
93109	2	399419	13	NULL	NULL	0	NULL	global transcriptional regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of global transcriptional regulation by ArcA , ArcB , Cra , Crp , Cya , Fnr , and Mlc on glucose catabolism in Escherichia coli .
	manualset3
93110	3	399419	13	NULL	NULL	0	NULL	ArcA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of global transcriptional regulation by ArcA , ArcB , Cra , Crp , Cya , Fnr , and Mlc on glucose catabolism in Escherichia coli .
	manualset3
93111	4	399419	13	NULL	NULL	0	NULL	ArcB	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of global transcriptional regulation by ArcA , ArcB , Cra , Crp , Cya , Fnr , and Mlc on glucose catabolism in Escherichia coli .
	manualset3
93112	5	399419	13	NULL	NULL	0	NULL	Cra	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of global transcriptional regulation by ArcA , ArcB , Cra , Crp , Cya , Fnr , and Mlc on glucose catabolism in Escherichia coli .
	manualset3
93113	6	399419	13	NULL	NULL	0	NULL	Crp	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of global transcriptional regulation by ArcA , ArcB , Cra , Crp , Cya , Fnr , and Mlc on glucose catabolism in Escherichia coli .
	manualset3
93114	7	399419	13	NULL	NULL	0	NULL	Cya	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of global transcriptional regulation by ArcA , ArcB , Cra , Crp , Cya , Fnr , and Mlc on glucose catabolism in Escherichia coli .
	manualset3
93115	8	399419	13	NULL	NULL	0	NULL	Fnr	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of global transcriptional regulation by ArcA , ArcB , Cra , Crp , Cya , Fnr , and Mlc on glucose catabolism in Escherichia coli .
	manualset3
93116	9	399419	13	NULL	NULL	0	NULL	Mlc	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of global transcriptional regulation by ArcA , ArcB , Cra , Crp , Cya , Fnr , and Mlc on glucose catabolism in Escherichia coli .
	manualset3
93117	10	399419	13	NULL	NULL	0	NULL	glucose catabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of global transcriptional regulation by ArcA , ArcB , Cra , Crp , Cya , Fnr , and Mlc on glucose catabolism in Escherichia coli .
	manualset3
93118	11	399419	13	NULL	NULL	0	NULL	Escherichia coli 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of global transcriptional regulation by ArcA , ArcB , Cra , Crp , Cya , Fnr , and Mlc on glucose catabolism in Escherichia coli .
	manualset3
93119	1	399420	13	NULL	NULL	0	NULL	Impact 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of heat stress exposure during meiotic maturation on oocyte , surrounding cumulus cell , and embryo RNA populations .
	manualset3
93120	2	399420	13	NULL	NULL	0	NULL	heat stress exposure	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of heat stress exposure during meiotic maturation on oocyte , surrounding cumulus cell , and embryo RNA populations .
	manualset3
93121	3	399420	13	NULL	NULL	0	NULL	meiotic maturation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of heat stress exposure during meiotic maturation on oocyte , surrounding cumulus cell , and embryo RNA populations .
	manualset3
93122	4	399420	13	NULL	NULL	0	NULL	 oocyte	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of heat stress exposure during meiotic maturation on oocyte , surrounding cumulus cell , and embryo RNA populations .
	manualset3
93123	5	399420	13	NULL	NULL	0	NULL	surrounding cumulus cell 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of heat stress exposure during meiotic maturation on oocyte , surrounding cumulus cell , and embryo RNA populations .
	manualset3
93124	6	399420	13	NULL	NULL	0	NULL	embryo RNA populations	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of heat stress exposure during meiotic maturation on oocyte , surrounding cumulus cell , and embryo RNA populations .
	manualset3
93125	1	399421	13	NULL	NULL	0	NULL	Impact	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of kidney cancer surgery on oncologic and kidney functional outcomes .
	manualset3
93126	2	399421	13	NULL	NULL	0	NULL	kidney cancer surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of kidney cancer surgery on oncologic and kidney functional outcomes .
	manualset3
93127	3	399421	13	NULL	NULL	0	NULL	oncologic outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of kidney cancer surgery on oncologic and kidney functional outcomes .
	manualset3
93128	4	399421	13	NULL	NULL	0	NULL	kidney functional outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of kidney cancer surgery on oncologic and kidney functional outcomes .
	manualset3
93129	1	399422	13	NULL	NULL	0	NULL	Impact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of mass media on adolescent sexual behavior : the chicken or the egg ? .
	manualset3
93130	2	399422	13	NULL	NULL	0	NULL	mass media 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of mass media on adolescent sexual behavior : the chicken or the egg ? .
	manualset3
93131	3	399422	13	NULL	NULL	0	NULL	adolescent sexual behavior	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of mass media on adolescent sexual behavior : the chicken or the egg ? .
	manualset3
93132	4	399422	13	NULL	NULL	0	NULL	chicken	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of mass media on adolescent sexual behavior : the chicken or the egg ? .
	manualset3
93133	5	399422	13	NULL	NULL	0	NULL	egg	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of mass media on adolescent sexual behavior : the chicken or the egg ? .
	manualset3
93134	1	399423	13	NULL	NULL	0	NULL	Impact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of omega-3 polyunsaturated fatty acids on coronary plaque instability : an integrated backscatter intravascular ultrasound study .
	manualset3
93135	2	399423	13	NULL	NULL	0	NULL	omega-3 polyunsaturated fatty acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of omega-3 polyunsaturated fatty acids on coronary plaque instability : an integrated backscatter intravascular ultrasound study .
	manualset3
93136	3	399423	13	NULL	NULL	0	NULL	coronary plaque instability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of omega-3 polyunsaturated fatty acids on coronary plaque instability : an integrated backscatter intravascular ultrasound study .
	manualset3
93137	4	399423	13	NULL	NULL	NULL	NULL	backscatter intravascular ultrasound study 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Impact of omega-3 polyunsaturated fatty acids on coronary plaque instability : an integrated backscatter intravascular ultrasound study .
	manualset3
93138	1	399424	13	NULL	NULL	0	NULL	Impact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of practice guidelines on support surface selection , incidence of pressure ulcers , and fiscal dollars .
	manualset3
93139	2	399424	13	NULL	NULL	0	NULL	practice guidelines	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of practice guidelines on support surface selection , incidence of pressure ulcers , and fiscal dollars .
	manualset3
93140	3	399424	13	NULL	NULL	0	NULL	support surface selection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of practice guidelines on support surface selection , incidence of pressure ulcers , and fiscal dollars .
	manualset3
93141	4	399424	13	NULL	NULL	0	NULL	incidence of pressure ulcers	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of practice guidelines on support surface selection , incidence of pressure ulcers , and fiscal dollars .
	manualset3
93142	5	399424	13	NULL	NULL	0	NULL	fiscal dollars	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of practice guidelines on support surface selection , incidence of pressure ulcers , and fiscal dollars .
	manualset3
93143	1	399425	13	NULL	NULL	0	NULL	Thoracic pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Thoracic pain caused by coronary insufficiency ) .
	manualset3
93144	2	399425	13	NULL	NULL	0	NULL	coronary insufficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Thoracic pain caused by coronary insufficiency ) .
	manualset3
93145	1	399426	13	NULL	NULL	0	NULL	Impact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of practitioner 's training in the management of alcohol dependence : a quasi-experimental 18-month follow-up study .
	manualset3
93146	2	399426	13	NULL	NULL	0	NULL	 practitioner 's	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of practitioner 's training in the management of alcohol dependence : a quasi-experimental 18-month follow-up study .
	manualset3
93147	3	399426	13	NULL	NULL	0	NULL	training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of practitioner 's training in the management of alcohol dependence : a quasi-experimental 18-month follow-up study .
	manualset3
93148	4	399426	13	NULL	NULL	0	NULL	 management of alcohol dependence	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Impact of practitioner 's training in the management of alcohol dependence : a quasi-experimental 18-month follow-up study .
	manualset3
93149	5	399426	13	NULL	NULL	NULL	NULL	a quasi-experimental 18-month follow-up study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Impact of practitioner 's training in the management of alcohol dependence : a quasi-experimental 18-month follow-up study .
	manualset3
93150	1	399427	13	NULL	NULL	NULL	NULL	cardiovascular responsiveness	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Impaired cardiovascular responsiveness in liver disease .
	manualset3
93151	2	399427	13	NULL	NULL	0	NULL	liver disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Impaired cardiovascular responsiveness in liver disease .
	manualset3
93152	1	399428	13	NULL	NULL	NULL	NULL	 catecholaminergic signalling	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Impaired catecholaminergic signalling of B lymphocytes in patients with chronic rheumatic diseases .
	manualset3
93153	2	399428	13	NULL	NULL	0	NULL	B lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Impaired catecholaminergic signalling of B lymphocytes in patients with chronic rheumatic diseases .
	manualset3
93154	3	399428	13	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Impaired catecholaminergic signalling of B lymphocytes in patients with chronic rheumatic diseases .
	manualset3
93155	4	399428	13	NULL	NULL	0	NULL	chronic rheumatic diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Impaired catecholaminergic signalling of B lymphocytes in patients with chronic rheumatic diseases .
	manualset3
93156	1	399429	13	NULL	NULL	NULL	NULL	dentofacial development 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Impaired dentofacial development after radiotherapy of a non-Hodgkin lymphoma : report of case .
	manualset3
93157	2	399429	13	NULL	NULL	0	NULL	 radiotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Impaired dentofacial development after radiotherapy of a non-Hodgkin lymphoma : report of case .
	manualset3
93158	3	399429	13	NULL	NULL	0	NULL	non-Hodgkin lymphoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Impaired dentofacial development after radiotherapy of a non-Hodgkin lymphoma : report of case .
	manualset3
93159	4	399429	13	NULL	NULL	0	NULL	report of case	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Impaired dentofacial development after radiotherapy of a non-Hodgkin lymphoma : report of case .
	manualset3
93160	1	399430	13	NULL	NULL	NULL	NULL	insulin binding	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Impaired insulin binding to isolated adipocytes in experimental diabetic ketoacidosis .
	manualset3
93161	2	399430	13	NULL	NULL	NULL	NULL	adipocytes	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Impaired insulin binding to isolated adipocytes in experimental diabetic ketoacidosis .
	manualset3
93162	3	399430	13	NULL	NULL	0	NULL	experimental diabetic ketoacidosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Impaired insulin binding to isolated adipocytes in experimental diabetic ketoacidosis .
	manualset3
93163	1	399431	13	NULL	NULL	0	NULL	Impairment determinations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Impairment determinations , return to work readiness , and wage replacement are unique components of medical services in the workers ' compensation system .
	manualset3
93164	2	399431	13	NULL	NULL	NULL	NULL	return to work readiness	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Impairment determinations , return to work readiness , and wage replacement are unique components of medical services in the workers ' compensation system .
	manualset3
93166	4	399431	13	NULL	NULL	0	NULL	wage replacement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Impairment determinations , return to work readiness , and wage replacement are unique components of medical services in the workers ' compensation system .
	manualset3
93167	5	399431	13	NULL	NULL	0	NULL	unique components	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Impairment determinations , return to work readiness , and wage replacement are unique components of medical services in the workers ' compensation system .
	manualset3
93168	6	399431	13	NULL	NULL	NULL	NULL	medical services	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Impairment determinations , return to work readiness , and wage replacement are unique components of medical services in the workers ' compensation system .
	manualset3
93169	7	399431	13	NULL	NULL	0	NULL	workers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Impairment determinations , return to work readiness , and wage replacement are unique components of medical services in the workers ' compensation system .
	manualset3
93170	8	399431	13	NULL	NULL	0	NULL	compensation system	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Impairment determinations , return to work readiness , and wage replacement are unique components of medical services in the workers ' compensation system .
	manualset3
93171	1	399432	13	NULL	NULL	0	NULL	Implementation of chemoprophylaxis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Implementation of chemoprophylaxis of leprosy in the Southern Marquesas with a single dose of 25 mg per kg rifampin .
	manualset3
93172	2	399432	13	NULL	NULL	0	NULL	 leprosy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Implementation of chemoprophylaxis of leprosy in the Southern Marquesas with a single dose of 25 mg per kg rifampin .
	manualset3
93173	3	399432	13	NULL	NULL	0	NULL	Southern Marquesas 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Implementation of chemoprophylaxis of leprosy in the Southern Marquesas with a single dose of 25 mg per kg rifampin .
	manualset3
93174	4	399432	13	NULL	NULL	0	NULL	single dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Implementation of chemoprophylaxis of leprosy in the Southern Marquesas with a single dose of 25 mg per kg rifampin .
	manualset3
93175	5	399432	13	NULL	NULL	0	NULL	25 mg per kg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Implementation of chemoprophylaxis of leprosy in the Southern Marquesas with a single dose of 25 mg per kg rifampin .
	manualset3
93176	6	399432	13	NULL	NULL	0	NULL	rifampin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Implementation of chemoprophylaxis of leprosy in the Southern Marquesas with a single dose of 25 mg per kg rifampin .
	manualset3
93177	1	399433	13	NULL	NULL	NULL	NULL	Implication	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Implication of the melanocortin-3 receptor in the regulation of food intake .
	manualset3
93178	2	399433	13	NULL	NULL	0	NULL	melanocortin-3 receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Implication of the melanocortin-3 receptor in the regulation of food intake .
	manualset3
93179	3	399433	13	NULL	NULL	0	NULL	regulation of food intake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Implication of the melanocortin-3 receptor in the regulation of food intake .
	manualset3
93180	1	399434	13	NULL	NULL	0	NULL	Implications 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Implications for IOR , object perception , and attentional capture are discussed .
	manualset3
93181	2	399434	13	NULL	NULL	0	NULL	IOR 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Implications for IOR , object perception , and attentional capture are discussed .
	manualset3
93182	3	399434	13	NULL	NULL	0	NULL	object perception	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Implications for IOR , object perception , and attentional capture are discussed .
	manualset3
93183	4	399434	13	NULL	NULL	0	NULL	attentional capture	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Implications for IOR , object perception , and attentional capture are discussed .
	manualset3
93184	1	399435	13	NULL	NULL	0	NULL	Implications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Implications for an evaluation of student drinking behaviors are discussed .
	manualset3
93185	2	399435	13	NULL	NULL	0	NULL	evaluation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Implications for an evaluation of student drinking behaviors are discussed .
	manualset3
93186	3	399435	13	NULL	NULL	0	NULL	student	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Implications for an evaluation of student drinking behaviors are discussed .
	manualset3
93187	4	399435	13	NULL	NULL	0	NULL	drinking behaviors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Implications for an evaluation of student drinking behaviors are discussed .
	manualset3
93188	1	399436	13	NULL	NULL	0	NULL	Implications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Implications for diagnosis of human neoplasms .
	manualset3
93189	2	399436	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Implications for diagnosis of human neoplasms .
	manualset3
93190	3	399436	13	NULL	NULL	0	NULL	human neoplasms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Implications for diagnosis of human neoplasms .
	manualset3
93191	1	399437	13	NULL	NULL	0	NULL	Implications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Implications for the design of integrated , multimedia , entertainment-education campaigns and integrated evaluation designs are discussed .
	manualset3
93192	2	399437	13	NULL	NULL	0	NULL	 design	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Implications for the design of integrated , multimedia , entertainment-education campaigns and integrated evaluation designs are discussed .
	manualset3
93193	3	399437	13	NULL	NULL	0	NULL	 multimedia	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Implications for the design of integrated , multimedia , entertainment-education campaigns and integrated evaluation designs are discussed .
	manualset3
93194	4	399437	13	NULL	NULL	0	NULL	entertainment-education campaigns 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Implications for the design of integrated , multimedia , entertainment-education campaigns and integrated evaluation designs are discussed .
	manualset3
93195	5	399437	13	NULL	NULL	0	NULL	evaluation designs	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Implications for the design of integrated , multimedia , entertainment-education campaigns and integrated evaluation designs are discussed .
	manualset3
93196	1	399438	13	NULL	NULL	0	NULL	Implicit overcompensation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Implicit overcompensation : the influence of negative self-instructions on performance of a self-paced motor task .
	manualset3
93197	2	399438	13	NULL	NULL	0	NULL	influence of negative self-instructions	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Implicit overcompensation : the influence of negative self-instructions on performance of a self-paced motor task .
	manualset3
93198	3	399438	13	NULL	NULL	0	NULL	performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Implicit overcompensation : the influence of negative self-instructions on performance of a self-paced motor task .
	manualset3
93199	4	399438	13	NULL	NULL	0	NULL	self-paced motor task 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Implicit overcompensation : the influence of negative self-instructions on performance of a self-paced motor task .
	manualset3
93200	1	399439	13	NULL	NULL	0	NULL	Importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Importance of sagittally reformatted images in CT evaluation of spondylolisthesis .
	manualset3
93201	2	399439	13	NULL	NULL	0	NULL	images	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Importance of sagittally reformatted images in CT evaluation of spondylolisthesis .
	manualset3
93202	3	399439	13	NULL	NULL	NULL	NULL	CT evaluation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Importance of sagittally reformatted images in CT evaluation of spondylolisthesis .
	manualset3
93203	4	399439	13	NULL	NULL	0	NULL	spondylolisthesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Importance of sagittally reformatted images in CT evaluation of spondylolisthesis .
	manualset3
93204	1	399440	13	NULL	NULL	0	NULL	Importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Importance of serum source for the in vitro replicative senescence of human bone marrow derived mesenchymal stem cells .
	manualset3
93205	2	399440	13	NULL	NULL	0	NULL	serum source	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Importance of serum source for the in vitro replicative senescence of human bone marrow derived mesenchymal stem cells .
	manualset3
93206	3	399440	13	NULL	NULL	0	NULL	replicative senescence 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Importance of serum source for the in vitro replicative senescence of human bone marrow derived mesenchymal stem cells .
	manualset3
93207	4	399440	13	NULL	NULL	0	NULL	human bone marrow derived mesenchymal stem cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Importance of serum source for the in vitro replicative senescence of human bone marrow derived mesenchymal stem cells .
	manualset3
93208	1	399441	13	NULL	NULL	0	NULL	Angiofibroma of nasal cavity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Angiofibroma of nasal cavity in a woman ) .
	manualset3
93209	2	399441	13	NULL	NULL	0	NULL	woman	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( Angiofibroma of nasal cavity in a woman ) .
	manualset3
93210	1	399442	13	NULL	NULL	0	NULL	Thoughts	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Thoughts on hypoproteinemia in surgery ) .
	manualset3
93211	2	399442	13	NULL	NULL	0	NULL	hypoproteinemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Thoughts on hypoproteinemia in surgery ) .
	manualset3
93212	3	399442	13	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Thoughts on hypoproteinemia in surgery ) .
	manualset3
93213	1	399443	13	NULL	NULL	0	NULL	Importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Importance of the carboxy-terminal 25 amino acid residues of lung collectins in interactions with lipids and alveolar type II cells .
	manualset3
93214	2	399443	13	NULL	NULL	0	NULL	carboxy-terminal 25 amino acid residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Importance of the carboxy-terminal 25 amino acid residues of lung collectins in interactions with lipids and alveolar type II cells .
	manualset3
93215	3	399443	13	NULL	NULL	0	NULL	lung collectins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Importance of the carboxy-terminal 25 amino acid residues of lung collectins in interactions with lipids and alveolar type II cells .
	manualset3
93216	4	399443	13	NULL	NULL	0	NULL	interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Importance of the carboxy-terminal 25 amino acid residues of lung collectins in interactions with lipids and alveolar type II cells .
	manualset3
93217	5	399443	13	NULL	NULL	0	NULL	lipids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Importance of the carboxy-terminal 25 amino acid residues of lung collectins in interactions with lipids and alveolar type II cells .
	manualset3
93218	6	399443	13	NULL	NULL	0	NULL	 alveolar type II cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Importance of the carboxy-terminal 25 amino acid residues of lung collectins in interactions with lipids and alveolar type II cells .
	manualset3
93219	1	399444	13	NULL	NULL	0	NULL	Important aspects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Important aspects of differential diagnosis are presented based on a study of the literature which should help the ENT specialist discriminate between hyperfunctional and hypofunctional dysphonia , which is very important for therapy .
	manualset3
93220	2	399444	13	NULL	NULL	0	NULL	 differential diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Important aspects of differential diagnosis are presented based on a study of the literature which should help the ENT specialist discriminate between hyperfunctional and hypofunctional dysphonia , which is very important for therapy .
	manualset3
93221	3	399444	13	NULL	NULL	0	NULL	study	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Important aspects of differential diagnosis are presented based on a study of the literature which should help the ENT specialist discriminate between hyperfunctional and hypofunctional dysphonia , which is very important for therapy .
	manualset3
93222	4	399444	13	NULL	NULL	0	NULL	literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Important aspects of differential diagnosis are presented based on a study of the literature which should help the ENT specialist discriminate between hyperfunctional and hypofunctional dysphonia , which is very important for therapy .
	manualset3
93223	5	399444	13	NULL	NULL	0	NULL	ENT specialist 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Important aspects of differential diagnosis are presented based on a study of the literature which should help the ENT specialist discriminate between hyperfunctional and hypofunctional dysphonia , which is very important for therapy .
	manualset3
93224	6	399444	13	NULL	NULL	0	NULL	hyperfunctional dysphonia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Important aspects of differential diagnosis are presented based on a study of the literature which should help the ENT specialist discriminate between hyperfunctional and hypofunctional dysphonia , which is very important for therapy .
	manualset3
93225	7	399444	13	NULL	NULL	0	NULL	hypofunctional dysphonia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Important aspects of differential diagnosis are presented based on a study of the literature which should help the ENT specialist discriminate between hyperfunctional and hypofunctional dysphonia , which is very important for therapy .
	manualset3
93226	8	399444	13	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Important aspects of differential diagnosis are presented based on a study of the literature which should help the ENT specialist discriminate between hyperfunctional and hypofunctional dysphonia , which is very important for therapy .
	manualset3
93227	1	399445	13	NULL	NULL	0	NULL	Important aspects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Important aspects of the dengue epidemics during the period 1995-2006 have been analyzed here , using epidemiological , clinical and laboratory data .
	manualset3
93228	2	399445	13	NULL	NULL	0	NULL	dengue epidemics	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Important aspects of the dengue epidemics during the period 1995-2006 have been analyzed here , using epidemiological , clinical and laboratory data .
	manualset3
93229	3	399445	13	NULL	NULL	0	NULL	period 1995-2006	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Important aspects of the dengue epidemics during the period 1995-2006 have been analyzed here , using epidemiological , clinical and laboratory data .
	manualset3
93230	4	399445	13	NULL	NULL	0	NULL	epidemiological data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Important aspects of the dengue epidemics during the period 1995-2006 have been analyzed here , using epidemiological , clinical and laboratory data .
	manualset3
93231	5	399445	13	NULL	NULL	0	NULL	clinical data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Important aspects of the dengue epidemics during the period 1995-2006 have been analyzed here , using epidemiological , clinical and laboratory data .
	manualset3
93232	6	399445	13	NULL	NULL	0	NULL	laboratory data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Important aspects of the dengue epidemics during the period 1995-2006 have been analyzed here , using epidemiological , clinical and laboratory data .
	manualset3
93233	1	399446	13	NULL	NULL	0	NULL	Important implications 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Important implications can be derived for the design and interpretation of experiments to characterize weak interactions , which are potentially important for brain processing .
	manualset3
93234	2	399446	13	NULL	NULL	NULL	NULL	design of experiments	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Important implications can be derived for the design and interpretation of experiments to characterize weak interactions , which are potentially important for brain processing .
	manualset3
93235	3	399446	13	NULL	NULL	0	NULL	interpretation of experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Important implications can be derived for the design and interpretation of experiments to characterize weak interactions , which are potentially important for brain processing .
	manualset3
93236	4	399446	13	NULL	NULL	NULL	NULL	 weak interactions	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Important implications can be derived for the design and interpretation of experiments to characterize weak interactions , which are potentially important for brain processing .
	manualset3
93237	5	399446	13	NULL	NULL	0	NULL	brain processing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Important implications can be derived for the design and interpretation of experiments to characterize weak interactions , which are potentially important for brain processing .
	manualset3
93238	1	399447	13	NULL	NULL	0	NULL	Important limitations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Important limitations of these vectors are that recombinant gene expression is transient and inflammation occurs at the site of gene transfer .
	manualset3
93239	2	399447	13	NULL	NULL	0	NULL	vectors	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Important limitations of these vectors are that recombinant gene expression is transient and inflammation occurs at the site of gene transfer .
	manualset3
93240	3	399447	13	NULL	NULL	0	NULL	recombinant gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Important limitations of these vectors are that recombinant gene expression is transient and inflammation occurs at the site of gene transfer .
	manualset3
93241	4	399447	13	NULL	NULL	0	NULL	inflammation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Important limitations of these vectors are that recombinant gene expression is transient and inflammation occurs at the site of gene transfer .
	manualset3
93242	5	399447	13	NULL	NULL	0	NULL	site of gene transfer 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Important limitations of these vectors are that recombinant gene expression is transient and inflammation occurs at the site of gene transfer .
	manualset3
93243	1	399448	13	NULL	NULL	0	NULL	Important pretreatment characteristics	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Important pretreatment characteristics that favor response are ambulatory status , female , less than 50 years old , no prior chemotherapy and no liver or brain metastases .
	manualset3
93244	2	399448	13	NULL	NULL	NULL	NULL	favor response	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Important pretreatment characteristics that favor response are ambulatory status , female , less than 50 years old , no prior chemotherapy and no liver or brain metastases .
	manualset3
93245	3	399448	13	NULL	NULL	0	NULL	ambulatory status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Important pretreatment characteristics that favor response are ambulatory status , female , less than 50 years old , no prior chemotherapy and no liver or brain metastases .
	manualset3
93246	4	399448	13	NULL	NULL	0	NULL	female	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Important pretreatment characteristics that favor response are ambulatory status , female , less than 50 years old , no prior chemotherapy and no liver or brain metastases .
	manualset3
93247	5	399448	13	NULL	NULL	0	NULL	less than 50 years old	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Important pretreatment characteristics that favor response are ambulatory status , female , less than 50 years old , no prior chemotherapy and no liver or brain metastases .
	manualset3
93248	6	399448	13	NULL	NULL	0	NULL	chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Important pretreatment characteristics that favor response are ambulatory status , female , less than 50 years old , no prior chemotherapy and no liver or brain metastases .
	manualset3
93249	7	399448	13	NULL	NULL	0	NULL	liver  metastases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Important pretreatment characteristics that favor response are ambulatory status , female , less than 50 years old , no prior chemotherapy and no liver or brain metastases .
	manualset3
93250	8	399448	13	NULL	NULL	0	NULL	brain metastases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Important pretreatment characteristics that favor response are ambulatory status , female , less than 50 years old , no prior chemotherapy and no liver or brain metastases .
	manualset3
93251	1	399449	13	NULL	NULL	0	NULL	Important risk factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Important risk factors for transmission of cholera were almost equally prevalent in the majority of both types of cholera cases .
	manualset3
93252	2	399449	13	NULL	NULL	0	NULL	transmission of cholera 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Important risk factors for transmission of cholera were almost equally prevalent in the majority of both types of cholera cases .
	manualset3
93253	3	399449	13	NULL	NULL	NULL	NULL	majority of both types of cholera cases	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Important risk factors for transmission of cholera were almost equally prevalent in the majority of both types of cholera cases .
	manualset3
93254	1	399450	13	NULL	NULL	0	NULL	HCV replicon replication	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , HCV replicon replication was efficiently inhibited by the allosteric ribozyme .
	manualset3
93255	2	399450	13	NULL	NULL	NULL	NULL	allosteric ribozyme	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Importantly , HCV replicon replication was efficiently inhibited by the allosteric ribozyme .
	manualset3
93256	1	399451	13	NULL	NULL	0	NULL	IC87114 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , IC87114 reduced cytokine production by memory T cells from healthy and allergic donors and from inflammatory arthritis patients .
	manualset3
93257	2	399451	13	NULL	NULL	0	NULL	cytokine production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , IC87114 reduced cytokine production by memory T cells from healthy and allergic donors and from inflammatory arthritis patients .
	manualset3
93258	3	399451	13	NULL	NULL	0	NULL	memory T cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , IC87114 reduced cytokine production by memory T cells from healthy and allergic donors and from inflammatory arthritis patients .
	manualset3
93259	4	399451	13	NULL	NULL	0	NULL	healthy donors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , IC87114 reduced cytokine production by memory T cells from healthy and allergic donors and from inflammatory arthritis patients .
	manualset3
93260	5	399451	13	NULL	NULL	0	NULL	allergic donors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , IC87114 reduced cytokine production by memory T cells from healthy and allergic donors and from inflammatory arthritis patients .
	manualset3
93261	6	399451	13	NULL	NULL	0	NULL	 inflammatory arthritis patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , IC87114 reduced cytokine production by memory T cells from healthy and allergic donors and from inflammatory arthritis patients .
	manualset3
93262	1	399452	13	NULL	NULL	0	NULL	Three dimensional analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Three dimensional analysis of noninvasive ductal carcinoma of the breast using immunohistochemical staining technique of laminin ) .
	manualset3
93263	2	399452	13	NULL	NULL	0	NULL	noninvasive ductal carcinoma of the breast	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Three dimensional analysis of noninvasive ductal carcinoma of the breast using immunohistochemical staining technique of laminin ) .
	manualset3
93264	3	399452	13	NULL	NULL	0	NULL	immunohistochemical staining technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Three dimensional analysis of noninvasive ductal carcinoma of the breast using immunohistochemical staining technique of laminin ) .
	manualset3
93265	4	399452	13	NULL	NULL	0	NULL	 laminin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Three dimensional analysis of noninvasive ductal carcinoma of the breast using immunohistochemical staining technique of laminin ) .
	manualset3
93266	1	399453	13	NULL	NULL	NULL	NULL	alternative pre-mRNA	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Importantly , alternative pre-mRNA splicing is kept under spatiotemporal control by circulating hormones and cellular activity , as well as being differentially modified during development and in different tissues .
	manualset3
93267	2	399453	13	NULL	NULL	0	NULL	spatiotemporal control 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , alternative pre-mRNA splicing is kept under spatiotemporal control by circulating hormones and cellular activity , as well as being differentially modified during development and in different tissues .
	manualset3
93268	3	399453	13	NULL	NULL	NULL	NULL	hormones	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Importantly , alternative pre-mRNA splicing is kept under spatiotemporal control by circulating hormones and cellular activity , as well as being differentially modified during development and in different tissues .
	manualset3
93269	4	399453	13	NULL	NULL	0	NULL	 cellular activity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , alternative pre-mRNA splicing is kept under spatiotemporal control by circulating hormones and cellular activity , as well as being differentially modified during development and in different tissues .
	manualset3
93270	5	399453	13	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , alternative pre-mRNA splicing is kept under spatiotemporal control by circulating hormones and cellular activity , as well as being differentially modified during development and in different tissues .
	manualset3
93271	6	399453	13	NULL	NULL	0	NULL	different tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , alternative pre-mRNA splicing is kept under spatiotemporal control by circulating hormones and cellular activity , as well as being differentially modified during development and in different tissues .
	manualset3
93272	1	399454	13	NULL	NULL	0	NULL	steatotic livers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , although steatotic livers were much more susceptible to IRI than lean livers , by most measures there was no statistical difference between the level of IRI to steatotic or lean livers when complement was inhibited .
	manualset3
93273	2	399454	13	NULL	NULL	0	NULL	IRI	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , although steatotic livers were much more susceptible to IRI than lean livers , by most measures there was no statistical difference between the level of IRI to steatotic or lean livers when complement was inhibited .
	manualset3
93274	3	399454	13	NULL	NULL	0	NULL	lean livers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , although steatotic livers were much more susceptible to IRI than lean livers , by most measures there was no statistical difference between the level of IRI to steatotic or lean livers when complement was inhibited .
	manualset3
93275	4	399454	13	NULL	NULL	0	NULL	measures	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , although steatotic livers were much more susceptible to IRI than lean livers , by most measures there was no statistical difference between the level of IRI to steatotic or lean livers when complement was inhibited .
	manualset3
93276	5	399454	13	NULL	NULL	0	NULL	statistical difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , although steatotic livers were much more susceptible to IRI than lean livers , by most measures there was no statistical difference between the level of IRI to steatotic or lean livers when complement was inhibited .
	manualset3
93277	6	399454	13	NULL	NULL	0	NULL	level of IRI	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , although steatotic livers were much more susceptible to IRI than lean livers , by most measures there was no statistical difference between the level of IRI to steatotic or lean livers when complement was inhibited .
	manualset3
93278	7	399454	13	NULL	NULL	0	NULL	steatotic livers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , although steatotic livers were much more susceptible to IRI than lean livers , by most measures there was no statistical difference between the level of IRI to steatotic or lean livers when complement was inhibited .
	manualset3
93279	8	399454	13	NULL	NULL	0	NULL	lean livers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , although steatotic livers were much more susceptible to IRI than lean livers , by most measures there was no statistical difference between the level of IRI to steatotic or lean livers when complement was inhibited .
	manualset3
93280	9	399454	13	NULL	NULL	0	NULL	complement	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , although steatotic livers were much more susceptible to IRI than lean livers , by most measures there was no statistical difference between the level of IRI to steatotic or lean livers when complement was inhibited .
	manualset3
93281	1	399455	13	NULL	NULL	0	NULL	genetic studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , genetic studies , as well as molecular cloning strategies , recently identified epithelial ion channels as the gatekeepers of active Ca2 + and Mg2 + reabsorption .
	manualset3
93282	2	399455	13	NULL	NULL	0	NULL	molecular cloning strategies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , genetic studies , as well as molecular cloning strategies , recently identified epithelial ion channels as the gatekeepers of active Ca2 + and Mg2 + reabsorption .
	manualset3
93283	3	399455	13	NULL	NULL	NULL	NULL	epithelial ion channels	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Importantly , genetic studies , as well as molecular cloning strategies , recently identified epithelial ion channels as the gatekeepers of active Ca2 + and Mg2 + reabsorption .
	manualset3
93284	4	399455	13	NULL	NULL	0	NULL	gatekeepers	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , genetic studies , as well as molecular cloning strategies , recently identified epithelial ion channels as the gatekeepers of active Ca2 + and Mg2 + reabsorption .
	manualset3
93285	5	399455	13	NULL	NULL	0	NULL	active Ca2 + reabsorption	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , genetic studies , as well as molecular cloning strategies , recently identified epithelial ion channels as the gatekeepers of active Ca2 + and Mg2 + reabsorption .
	manualset3
93286	6	399455	13	NULL	NULL	0	NULL	active Mg2 + reabsorption	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , genetic studies , as well as molecular cloning strategies , recently identified epithelial ion channels as the gatekeepers of active Ca2 + and Mg2 + reabsorption .
	manualset3
93342	2	399456	13	NULL	NULL	NULL	NULL	 Golgi fragmentation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Importantly , in addition to Golgi fragmentation , increased F-actin content in the absence of FMNL1 also led to cation-independent mannose 6-phosphate receptor dispersal , lysosomal enlargement and missorting of cathepsin D. Taken together , our data support a model in which FMNL1 regulates cellular F-actin levels required to maintain structural integrity of the Golgi complex and lysosomes .
	manualset3
93343	3	399456	13	NULL	NULL	NULL	NULL	F-actin content	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Importantly , in addition to Golgi fragmentation , increased F-actin content in the absence of FMNL1 also led to cation-independent mannose 6-phosphate receptor dispersal , lysosomal enlargement and missorting of cathepsin D. Taken together , our data support a model in which FMNL1 regulates cellular F-actin levels required to maintain structural integrity of the Golgi complex and lysosomes .
	manualset3
93344	5	399456	13	NULL	NULL	NULL	NULL	FMNL1 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Importantly , in addition to Golgi fragmentation , increased F-actin content in the absence of FMNL1 also led to cation-independent mannose 6-phosphate receptor dispersal , lysosomal enlargement and missorting of cathepsin D. Taken together , our data support a model in which FMNL1 regulates cellular F-actin levels required to maintain structural integrity of the Golgi complex and lysosomes .
	manualset3
93345	6	399456	13	NULL	NULL	NULL	NULL	cation-independent mannose 6-phosphate receptor dispersal	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Importantly , in addition to Golgi fragmentation , increased F-actin content in the absence of FMNL1 also led to cation-independent mannose 6-phosphate receptor dispersal , lysosomal enlargement and missorting of cathepsin D. Taken together , our data support a model in which FMNL1 regulates cellular F-actin levels required to maintain structural integrity of the Golgi complex and lysosomes .
	manualset3
93346	7	399456	13	NULL	NULL	NULL	NULL	 lysosomal enlargement	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Importantly , in addition to Golgi fragmentation , increased F-actin content in the absence of FMNL1 also led to cation-independent mannose 6-phosphate receptor dispersal , lysosomal enlargement and missorting of cathepsin D. Taken together , our data support a model in which FMNL1 regulates cellular F-actin levels required to maintain structural integrity of the Golgi complex and lysosomes .
	manualset3
93347	8	399456	13	NULL	NULL	NULL	NULL	cathepsin D	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Importantly , in addition to Golgi fragmentation , increased F-actin content in the absence of FMNL1 also led to cation-independent mannose 6-phosphate receptor dispersal , lysosomal enlargement and missorting of cathepsin D. Taken together , our data support a model in which FMNL1 regulates cellular F-actin levels required to maintain structural integrity of the Golgi complex and lysosomes .
	manualset3
93348	9	399456	13	NULL	NULL	NULL	NULL	data 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Importantly , in addition to Golgi fragmentation , increased F-actin content in the absence of FMNL1 also led to cation-independent mannose 6-phosphate receptor dispersal , lysosomal enlargement and missorting of cathepsin D. Taken together , our data support a model in which FMNL1 regulates cellular F-actin levels required to maintain structural integrity of the Golgi complex and lysosomes .
	manualset3
93349	10	399456	13	NULL	NULL	NULL	NULL	 model	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Importantly , in addition to Golgi fragmentation , increased F-actin content in the absence of FMNL1 also led to cation-independent mannose 6-phosphate receptor dispersal , lysosomal enlargement and missorting of cathepsin D. Taken together , our data support a model in which FMNL1 regulates cellular F-actin levels required to maintain structural integrity of the Golgi complex and lysosomes .
	manualset3
93350	11	399456	13	NULL	NULL	NULL	NULL	FMNL1 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Importantly , in addition to Golgi fragmentation , increased F-actin content in the absence of FMNL1 also led to cation-independent mannose 6-phosphate receptor dispersal , lysosomal enlargement and missorting of cathepsin D. Taken together , our data support a model in which FMNL1 regulates cellular F-actin levels required to maintain structural integrity of the Golgi complex and lysosomes .
	manualset3
93352	12	399456	13	NULL	NULL	NULL	NULL	cellular F-actin levels	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Importantly , in addition to Golgi fragmentation , increased F-actin content in the absence of FMNL1 also led to cation-independent mannose 6-phosphate receptor dispersal , lysosomal enlargement and missorting of cathepsin D. Taken together , our data support a model in which FMNL1 regulates cellular F-actin levels required to maintain structural integrity of the Golgi complex and lysosomes .
	manualset3
93353	13	399456	13	NULL	NULL	NULL	NULL	structural integrity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Importantly , in addition to Golgi fragmentation , increased F-actin content in the absence of FMNL1 also led to cation-independent mannose 6-phosphate receptor dispersal , lysosomal enlargement and missorting of cathepsin D. Taken together , our data support a model in which FMNL1 regulates cellular F-actin levels required to maintain structural integrity of the Golgi complex and lysosomes .
	manualset3
93354	13	399456	13	NULL	NULL	0	NULL	Golgi complex	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , in addition to Golgi fragmentation , increased F-actin content in the absence of FMNL1 also led to cation-independent mannose 6-phosphate receptor dispersal , lysosomal enlargement and missorting of cathepsin D. Taken together , our data support a model in which FMNL1 regulates cellular F-actin levels required to maintain structural integrity of the Golgi complex and lysosomes .
	manualset3
93355	14	399456	13	NULL	NULL	0	NULL	lysosomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , in addition to Golgi fragmentation , increased F-actin content in the absence of FMNL1 also led to cation-independent mannose 6-phosphate receptor dispersal , lysosomal enlargement and missorting of cathepsin D. Taken together , our data support a model in which FMNL1 regulates cellular F-actin levels required to maintain structural integrity of the Golgi complex and lysosomes .
	manualset3
93356	1	399456	13	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , in addition to Golgi fragmentation , increased F-actin content in the absence of FMNL1 also led to cation-independent mannose 6-phosphate receptor dispersal , lysosomal enlargement and missorting of cathepsin D. Taken together , our data support a model in which FMNL1 regulates cellular F-actin levels required to maintain structural integrity of the Golgi complex and lysosomes .
	manualset3
93357	4	399456	13	NULL	NULL	0	NULL	 absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , in addition to Golgi fragmentation , increased F-actin content in the absence of FMNL1 also led to cation-independent mannose 6-phosphate receptor dispersal , lysosomal enlargement and missorting of cathepsin D. Taken together , our data support a model in which FMNL1 regulates cellular F-actin levels required to maintain structural integrity of the Golgi complex and lysosomes .
	manualset3
93358	1	399457	13	NULL	NULL	0	NULL	 results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , our results establish the enhanced antitumor activity in vivo of the i-leader C-terminal truncated mutants , especially in a desmotic fibroblast-embedded lung carcinoma model in mice .
	manualset3
93359	2	399457	13	NULL	NULL	0	NULL	antitumor activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , our results establish the enhanced antitumor activity in vivo of the i-leader C-terminal truncated mutants , especially in a desmotic fibroblast-embedded lung carcinoma model in mice .
	manualset3
93360	3	399457	13	NULL	NULL	0	NULL	i-leader C-terminal truncated mutants	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , our results establish the enhanced antitumor activity in vivo of the i-leader C-terminal truncated mutants , especially in a desmotic fibroblast-embedded lung carcinoma model in mice .
	manualset3
93361	4	399457	13	NULL	NULL	0	NULL	desmotic fibroblast-embedded lung carcinoma model	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , our results establish the enhanced antitumor activity in vivo of the i-leader C-terminal truncated mutants , especially in a desmotic fibroblast-embedded lung carcinoma model in mice .
	manualset3
93362	5	399457	13	NULL	NULL	0	NULL	mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , our results establish the enhanced antitumor activity in vivo of the i-leader C-terminal truncated mutants , especially in a desmotic fibroblast-embedded lung carcinoma model in mice .
	manualset3
93363	1	399458	13	NULL	NULL	0	NULL	platelet adhesiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , platelet adhesiveness , abnormal before treatment 77.2 + / - 1.3 % ( normal less than 70 % ) , improved throughout the study to 57.8 + / - 1.3 % after 36 months of gliclazide .
	manualset3
93364	2	399458	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , platelet adhesiveness , abnormal before treatment 77.2 + / - 1.3 % ( normal less than 70 % ) , improved throughout the study to 57.8 + / - 1.3 % after 36 months of gliclazide .
	manualset3
93365	3	399458	13	NULL	NULL	0	NULL	77.2 + / - 1.3 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , platelet adhesiveness , abnormal before treatment 77.2 + / - 1.3 % ( normal less than 70 % ) , improved throughout the study to 57.8 + / - 1.3 % after 36 months of gliclazide .
	manualset3
93366	4	399458	13	NULL	NULL	0	NULL	normal less than 70 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , platelet adhesiveness , abnormal before treatment 77.2 + / - 1.3 % ( normal less than 70 % ) , improved throughout the study to 57.8 + / - 1.3 % after 36 months of gliclazide .
	manualset3
93367	5	399458	13	NULL	NULL	0	NULL	study	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , platelet adhesiveness , abnormal before treatment 77.2 + / - 1.3 % ( normal less than 70 % ) , improved throughout the study to 57.8 + / - 1.3 % after 36 months of gliclazide .
	manualset3
93368	6	399458	13	NULL	NULL	0	NULL	57.8 + / - 1.3 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , platelet adhesiveness , abnormal before treatment 77.2 + / - 1.3 % ( normal less than 70 % ) , improved throughout the study to 57.8 + / - 1.3 % after 36 months of gliclazide .
	manualset3
93369	7	399458	13	NULL	NULL	0	NULL	 36 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , platelet adhesiveness , abnormal before treatment 77.2 + / - 1.3 % ( normal less than 70 % ) , improved throughout the study to 57.8 + / - 1.3 % after 36 months of gliclazide .
	manualset3
93370	8	399458	13	NULL	NULL	0	NULL	gliclazide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , platelet adhesiveness , abnormal before treatment 77.2 + / - 1.3 % ( normal less than 70 % ) , improved throughout the study to 57.8 + / - 1.3 % after 36 months of gliclazide .
	manualset3
93371	1	399459	13	NULL	NULL	0	NULL	 quinupristin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , quinupristin/dalfopristin shows similar activity against methicillin-susceptible and - resistant strains of S. aureus , and streptococci with benzylpenicillin ( penicillin G ) - or erythromycin-acquired resistance .
	manualset3
93372	2	399459	13	NULL	NULL	0	NULL	dalfopristin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , quinupristin/dalfopristin shows similar activity against methicillin-susceptible and - resistant strains of S. aureus , and streptococci with benzylpenicillin ( penicillin G ) - or erythromycin-acquired resistance .
	manualset3
93373	3	399459	13	NULL	NULL	0	NULL	 activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , quinupristin/dalfopristin shows similar activity against methicillin-susceptible and - resistant strains of S. aureus , and streptococci with benzylpenicillin ( penicillin G ) - or erythromycin-acquired resistance .
	manualset3
93374	4	399459	13	NULL	NULL	0	NULL	methicillin-susceptible strains of S. aureus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , quinupristin/dalfopristin shows similar activity against methicillin-susceptible and - resistant strains of S. aureus , and streptococci with benzylpenicillin ( penicillin G ) - or erythromycin-acquired resistance .
	manualset3
93375	5	399459	13	NULL	NULL	0	NULL	 methicillin- resistant strains of S. aureus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , quinupristin/dalfopristin shows similar activity against methicillin-susceptible and - resistant strains of S. aureus , and streptococci with benzylpenicillin ( penicillin G ) - or erythromycin-acquired resistance .
	manualset3
93376	6	399459	13	NULL	NULL	0	NULL	streptococci	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , quinupristin/dalfopristin shows similar activity against methicillin-susceptible and - resistant strains of S. aureus , and streptococci with benzylpenicillin ( penicillin G ) - or erythromycin-acquired resistance .
	manualset3
93377	7	399459	13	NULL	NULL	0	NULL	benzylpenicillin ( penicillin G )-acquired resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , quinupristin/dalfopristin shows similar activity against methicillin-susceptible and - resistant strains of S. aureus , and streptococci with benzylpenicillin ( penicillin G ) - or erythromycin-acquired resistance .
	manualset3
93378	8	399459	13	NULL	NULL	0	NULL	erythromycin-acquired resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , quinupristin/dalfopristin shows similar activity against methicillin-susceptible and - resistant strains of S. aureus , and streptococci with benzylpenicillin ( penicillin G ) - or erythromycin-acquired resistance .
	manualset3
93379	1	399460	13	NULL	NULL	0	NULL	Ets2 ( A72/A72 ) allele 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , the Ets2 ( A72/A72 ) allele resulted in decreased expression of inflammatory response genes , including TNF-alpha , CCL3 , matrix metalloprotease 9 , integrin alpha ( M ) , and Bcl-X in alveolar macrophage .
	manualset3
93380	2	399460	13	NULL	NULL	0	NULL	 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , the Ets2 ( A72/A72 ) allele resulted in decreased expression of inflammatory response genes , including TNF-alpha , CCL3 , matrix metalloprotease 9 , integrin alpha ( M ) , and Bcl-X in alveolar macrophage .
	manualset3
93381	3	399460	13	NULL	NULL	0	NULL	 inflammatory response genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , the Ets2 ( A72/A72 ) allele resulted in decreased expression of inflammatory response genes , including TNF-alpha , CCL3 , matrix metalloprotease 9 , integrin alpha ( M ) , and Bcl-X in alveolar macrophage .
	manualset3
93382	4	399460	13	NULL	NULL	0	NULL	TNF-alpha	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , the Ets2 ( A72/A72 ) allele resulted in decreased expression of inflammatory response genes , including TNF-alpha , CCL3 , matrix metalloprotease 9 , integrin alpha ( M ) , and Bcl-X in alveolar macrophage .
	manualset3
93383	5	399460	13	NULL	NULL	0	NULL	CCL3	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , the Ets2 ( A72/A72 ) allele resulted in decreased expression of inflammatory response genes , including TNF-alpha , CCL3 , matrix metalloprotease 9 , integrin alpha ( M ) , and Bcl-X in alveolar macrophage .
	manualset3
93384	6	399460	13	NULL	NULL	0	NULL	 matrix metalloprotease 9	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , the Ets2 ( A72/A72 ) allele resulted in decreased expression of inflammatory response genes , including TNF-alpha , CCL3 , matrix metalloprotease 9 , integrin alpha ( M ) , and Bcl-X in alveolar macrophage .
	manualset3
93385	7	399460	13	NULL	NULL	0	NULL	integrin alpha ( M )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , the Ets2 ( A72/A72 ) allele resulted in decreased expression of inflammatory response genes , including TNF-alpha , CCL3 , matrix metalloprotease 9 , integrin alpha ( M ) , and Bcl-X in alveolar macrophage .
	manualset3
93386	8	399460	13	NULL	NULL	0	NULL	Bcl-X	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , the Ets2 ( A72/A72 ) allele resulted in decreased expression of inflammatory response genes , including TNF-alpha , CCL3 , matrix metalloprotease 9 , integrin alpha ( M ) , and Bcl-X in alveolar macrophage .
	manualset3
93387	9	399460	13	NULL	NULL	0	NULL	alveolar macrophage	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , the Ets2 ( A72/A72 ) allele resulted in decreased expression of inflammatory response genes , including TNF-alpha , CCL3 , matrix metalloprotease 9 , integrin alpha ( M ) , and Bcl-X in alveolar macrophage .
	manualset3
93388	1	399461	13	NULL	NULL	0	NULL	XOR inhibitors	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , the XOR inhibitors allopurinol and oxypurinol attenuate dysfunction caused by XOR in these disease states .
	manualset3
93389	2	399461	13	NULL	NULL	0	NULL	allopurinol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , the XOR inhibitors allopurinol and oxypurinol attenuate dysfunction caused by XOR in these disease states .
	manualset3
93390	3	399461	13	NULL	NULL	0	NULL	oxypurinol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , the XOR inhibitors allopurinol and oxypurinol attenuate dysfunction caused by XOR in these disease states .
	manualset3
93391	4	399461	13	NULL	NULL	0	NULL	dysfunction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , the XOR inhibitors allopurinol and oxypurinol attenuate dysfunction caused by XOR in these disease states .
	manualset3
93392	5	399461	13	NULL	NULL	0	NULL	XOR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , the XOR inhibitors allopurinol and oxypurinol attenuate dysfunction caused by XOR in these disease states .
	manualset3
93393	6	399461	13	NULL	NULL	0	NULL	disease states	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , the XOR inhibitors allopurinol and oxypurinol attenuate dysfunction caused by XOR in these disease states .
	manualset3
93394	1	399462	13	NULL	NULL	0	NULL	siRNA-mediated reduction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , the siRNA-mediated reduction in cyclins resulted in decreased IC ( 50 ) ( 50 % inhibitory concentration ) values for both doxorubicin and etoposide .
	manualset3
93395	2	399462	13	NULL	NULL	0	NULL	cyclins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , the siRNA-mediated reduction in cyclins resulted in decreased IC ( 50 ) ( 50 % inhibitory concentration ) values for both doxorubicin and etoposide .
	manualset3
93396	3	399462	13	NULL	NULL	NULL	NULL	IC ( 50 ) values	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Importantly , the siRNA-mediated reduction in cyclins resulted in decreased IC ( 50 ) ( 50 % inhibitory concentration ) values for both doxorubicin and etoposide .
	manualset3
93397	4	399462	13	NULL	NULL	0	NULL	50 % inhibitory concentration	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , the siRNA-mediated reduction in cyclins resulted in decreased IC ( 50 ) ( 50 % inhibitory concentration ) values for both doxorubicin and etoposide .
	manualset3
93398	5	399462	13	NULL	NULL	0	NULL	doxorubicin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , the siRNA-mediated reduction in cyclins resulted in decreased IC ( 50 ) ( 50 % inhibitory concentration ) values for both doxorubicin and etoposide .
	manualset3
93399	6	399462	13	NULL	NULL	0	NULL	etoposide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , the siRNA-mediated reduction in cyclins resulted in decreased IC ( 50 ) ( 50 % inhibitory concentration ) values for both doxorubicin and etoposide .
	manualset3
93400	1	399463	13	NULL	NULL	0	NULL	undifferentiated ASCs 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , we also show that undifferentiated ASCs and ASC-derived hepatic cells engraft robustly into the liver in a mouse model of toxic injury .
	manualset3
93401	2	399463	13	NULL	NULL	0	NULL	ASC-derived hepatic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , we also show that undifferentiated ASCs and ASC-derived hepatic cells engraft robustly into the liver in a mouse model of toxic injury .
	manualset3
93402	3	399463	13	NULL	NULL	0	NULL	 liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , we also show that undifferentiated ASCs and ASC-derived hepatic cells engraft robustly into the liver in a mouse model of toxic injury .
	manualset3
93403	4	399463	13	NULL	NULL	0	NULL	mouse model 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , we also show that undifferentiated ASCs and ASC-derived hepatic cells engraft robustly into the liver in a mouse model of toxic injury .
	manualset3
93404	5	399463	13	NULL	NULL	0	NULL	 toxic injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , we also show that undifferentiated ASCs and ASC-derived hepatic cells engraft robustly into the liver in a mouse model of toxic injury .
	manualset3
93405	1	399464	13	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , we identify a role for endogenous Smac in overcoming XIAP to allow myotube death .
	manualset3
93406	2	399464	13	NULL	NULL	0	NULL	endogenous Smac	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , we identify a role for endogenous Smac in overcoming XIAP to allow myotube death .
	manualset3
93407	3	399464	13	NULL	NULL	0	NULL	XIAP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , we identify a role for endogenous Smac in overcoming XIAP to allow myotube death .
	manualset3
93408	4	399464	13	NULL	NULL	0	NULL	myotube death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Importantly , we identify a role for endogenous Smac in overcoming XIAP to allow myotube death .
	manualset3
93409	1	399465	13	NULL	NULL	0	NULL	prior studies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Importing prior studies is best performed by creating a new order on the institution 's imaging system and then associating the DICOM objects from the prior study with it .
	manualset3
93410	2	399465	13	NULL	NULL	0	NULL	new order	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Importing prior studies is best performed by creating a new order on the institution 's imaging system and then associating the DICOM objects from the prior study with it .
	manualset3
93411	3	399465	13	NULL	NULL	0	NULL	 institution 's imaging system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Importing prior studies is best performed by creating a new order on the institution 's imaging system and then associating the DICOM objects from the prior study with it .
	manualset3
93412	4	399465	13	NULL	NULL	0	NULL	DICOM objects	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Importing prior studies is best performed by creating a new order on the institution 's imaging system and then associating the DICOM objects from the prior study with it .
	manualset3
93413	5	399465	13	NULL	NULL	0	NULL	 prior study 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Importing prior studies is best performed by creating a new order on the institution 's imaging system and then associating the DICOM objects from the prior study with it .
	manualset3
93414	1	399466	13	NULL	NULL	0	NULL	Impressions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Impressions of plastic and maxillo-facial surgery in the Palestine war .
	manualset3
93415	2	399466	13	NULL	NULL	0	NULL	plastic surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Impressions of plastic and maxillo-facial surgery in the Palestine war .
	manualset3
93416	3	399466	13	NULL	NULL	0	NULL	maxillo-facial surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Impressions of plastic and maxillo-facial surgery in the Palestine war .
	manualset3
93417	4	399466	13	NULL	NULL	0	NULL	Palestine war 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Impressions of plastic and maxillo-facial surgery in the Palestine war .
	manualset3
93418	1	399467	13	NULL	NULL	0	NULL	Impressions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Impressions were obtained with polyvinyl siloxane , and replicas were fabricated with the use of polyether impression material .
	manualset3
93419	2	399467	13	NULL	NULL	0	NULL	polyvinyl siloxane	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Impressions were obtained with polyvinyl siloxane , and replicas were fabricated with the use of polyether impression material .
	manualset3
93420	3	399467	13	NULL	NULL	0	NULL	replicas 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Impressions were obtained with polyvinyl siloxane , and replicas were fabricated with the use of polyether impression material .
	manualset3
93421	4	399467	13	NULL	NULL	0	NULL	polyether impression material	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Impressions were obtained with polyvinyl siloxane , and replicas were fabricated with the use of polyether impression material .
	manualset3
93422	5	399467	13	NULL	NULL	0	NULL	 use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Impressions were obtained with polyvinyl siloxane , and replicas were fabricated with the use of polyether impression material .
	manualset3
93423	1	399468	13	NULL	NULL	0	NULL	practice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Improve your practice with effective telephone management .
	manualset3
93424	2	399468	13	NULL	NULL	0	NULL	telephone management 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Improve your practice with effective telephone management .
	manualset3
93425	1	399469	13	NULL	NULL	0	NULL	hearing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Improved hearing was documented in 15 cases .
	manualset3
93426	2	399469	13	NULL	NULL	0	NULL	15 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Improved hearing was documented in 15 cases .
	manualset3
93427	1	399470	13	NULL	NULL	0	NULL	Thrombendarterectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Thrombendarterectomy of the carotid artery in the prevention of cerebrovascular insult ) .
	manualset3
93428	2	399470	13	NULL	NULL	0	NULL	 carotid artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Thrombendarterectomy of the carotid artery in the prevention of cerebrovascular insult ) .
	manualset3
93429	3	399470	13	NULL	NULL	0	NULL	prevention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Thrombendarterectomy of the carotid artery in the prevention of cerebrovascular insult ) .
	manualset3
93430	4	399470	13	NULL	NULL	0	NULL	cerebrovascular insult 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Thrombendarterectomy of the carotid artery in the prevention of cerebrovascular insult ) .
	manualset3
93431	1	399471	13	NULL	NULL	0	NULL	pectinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Improved pectinase production in Penicillium griseoroseum recombinant strains .
	manualset3
93432	2	399471	13	NULL	NULL	0	NULL	production 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Improved pectinase production in Penicillium griseoroseum recombinant strains .
	manualset3
93433	3	399471	13	NULL	NULL	0	NULL	Penicillium griseoroseum recombinant strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Improved pectinase production in Penicillium griseoroseum recombinant strains .
	manualset3
93434	1	399472	13	NULL	NULL	0	NULL	 procedures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Improved procedures for purification of the Bandeiraea simplicifolia I isolectins and Bandeiraea simplicifolia II lectin by affinity chromatography .
	manualset3
93435	2	399472	13	NULL	NULL	0	NULL	purification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Improved procedures for purification of the Bandeiraea simplicifolia I isolectins and Bandeiraea simplicifolia II lectin by affinity chromatography .
	manualset3
93436	3	399472	13	NULL	NULL	0	NULL	Bandeiraea simplicifolia I isolectins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Improved procedures for purification of the Bandeiraea simplicifolia I isolectins and Bandeiraea simplicifolia II lectin by affinity chromatography .
	manualset3
93437	4	399472	13	NULL	NULL	0	NULL	Bandeiraea simplicifolia II lectin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Improved procedures for purification of the Bandeiraea simplicifolia I isolectins and Bandeiraea simplicifolia II lectin by affinity chromatography .
	manualset3
93438	5	399472	13	NULL	NULL	0	NULL	affinity chromatography 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Improved procedures for purification of the Bandeiraea simplicifolia I isolectins and Bandeiraea simplicifolia II lectin by affinity chromatography .
	manualset3
93439	1	399473	13	NULL	NULL	0	NULL	Improvement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Improvement of malt modification by use of Rhizopus VII as starter culture .
	manualset3
93440	2	399473	13	NULL	NULL	0	NULL	malt modification 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Improvement of malt modification by use of Rhizopus VII as starter culture .
	manualset3
93441	3	399473	13	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Improvement of malt modification by use of Rhizopus VII as starter culture .
	manualset3
93442	4	399473	13	NULL	NULL	0	NULL	 Rhizopus VII	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Improvement of malt modification by use of Rhizopus VII as starter culture .
	manualset3
93443	5	399473	13	NULL	NULL	0	NULL	starter culture	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Improvement of malt modification by use of Rhizopus VII as starter culture .
	manualset3
93444	1	399474	13	NULL	NULL	0	NULL	access	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Improving access to palliative care through an innovative quality improvement initiative : an opportunity for pay-for-performance .
	manualset3
93445	2	399474	13	NULL	NULL	NULL	NULL	palliative care	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Improving access to palliative care through an innovative quality improvement initiative : an opportunity for pay-for-performance .
	manualset3
93446	3	399474	13	NULL	NULL	0	NULL	 quality improvement initiative	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Improving access to palliative care through an innovative quality improvement initiative : an opportunity for pay-for-performance .
	manualset3
93447	4	399474	13	NULL	NULL	0	NULL	opportunity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Improving access to palliative care through an innovative quality improvement initiative : an opportunity for pay-for-performance .
	manualset3
93448	5	399474	13	NULL	NULL	0	NULL	pay-for-performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Improving access to palliative care through an innovative quality improvement initiative : an opportunity for pay-for-performance .
	manualset3
93449	1	399475	13	NULL	NULL	0	NULL	clearance	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Improving clearance of the mutant protein is expected to prevent cellular dysfunction and neurodegeneration in HD .
	manualset3
93450	2	399475	13	NULL	NULL	0	NULL	mutant protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Improving clearance of the mutant protein is expected to prevent cellular dysfunction and neurodegeneration in HD .
	manualset3
93451	3	399475	13	NULL	NULL	0	NULL	 cellular dysfunction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Improving clearance of the mutant protein is expected to prevent cellular dysfunction and neurodegeneration in HD .
	manualset3
93452	4	399475	13	NULL	NULL	0	NULL	neurodegeneration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Improving clearance of the mutant protein is expected to prevent cellular dysfunction and neurodegeneration in HD .
	manualset3
93453	5	399475	13	NULL	NULL	0	NULL	HD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Improving clearance of the mutant protein is expected to prevent cellular dysfunction and neurodegeneration in HD .
	manualset3
93454	1	399476	13	NULL	NULL	0	NULL	Thrombocytosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Thrombocytosis in ulcerative colitis and regional enteritis ) .
	manualset3
93455	2	399476	13	NULL	NULL	0	NULL	ulcerative colitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Thrombocytosis in ulcerative colitis and regional enteritis ) .
	manualset3
93456	3	399476	13	NULL	NULL	0	NULL	regional enteritis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Thrombocytosis in ulcerative colitis and regional enteritis ) .
	manualset3
93457	1	399477	13	NULL	NULL	0	NULL	follow-up	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Improving the follow-up of positive hemoccult screening tests : an electronic intervention .
	manualset3
93458	2	399477	13	NULL	NULL	0	NULL	hemoccult screening tests	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Improving the follow-up of positive hemoccult screening tests : an electronic intervention .
	manualset3
93459	3	399477	13	NULL	NULL	0	NULL	electronic intervention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Improving the follow-up of positive hemoccult screening tests : an electronic intervention .
	manualset3
93460	1	399478	13	NULL	NULL	0	NULL	workforce	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Improving workforce is crucial to viability of Europe 's health services , commission says .
	manualset3
93461	2	399478	13	NULL	NULL	0	NULL	 viability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Improving workforce is crucial to viability of Europe 's health services , commission says .
	manualset3
93462	3	399478	13	NULL	NULL	0	NULL	Europe 's health services	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Improving workforce is crucial to viability of Europe 's health services , commission says .
	manualset3
93463	4	399478	13	NULL	NULL	0	NULL	 commission	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Improving workforce is crucial to viability of Europe 's health services , commission says .
	manualset3
93464	1	399479	13	NULL	NULL	NULL	NULL	Impulsiveness	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Impulsiveness and the prolactin response to d-fenfluramine .
	manualset3
93465	2	399479	13	NULL	NULL	0	NULL	 prolactin response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Impulsiveness and the prolactin response to d-fenfluramine .
	manualset3
93466	3	399479	13	NULL	NULL	0	NULL	d-fenfluramine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Impulsiveness and the prolactin response to d-fenfluramine .
	manualset3
93467	1	399480	13	NULL	NULL	0	NULL	ImuVert 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	ImuVert , a biologic response modifier , is capable of activating mononuclear cells causing release of various cytokines .
	manualset3
93468	2	399480	13	NULL	NULL	0	NULL	biologic response modifier	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	ImuVert , a biologic response modifier , is capable of activating mononuclear cells causing release of various cytokines .
	manualset3
93469	3	399480	13	NULL	NULL	0	NULL	 mononuclear cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	ImuVert , a biologic response modifier , is capable of activating mononuclear cells causing release of various cytokines .
	manualset3
93470	4	399480	13	NULL	NULL	0	NULL	release of various cytokines 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	ImuVert , a biologic response modifier , is capable of activating mononuclear cells causing release of various cytokines .
	manualset3
93471	1	399481	13	NULL	NULL	0	NULL	In-stent restenosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In-stent restenosis , thrombosis , and aneurysm formation are known complications .
	manualset3
93472	2	399481	13	NULL	NULL	0	NULL	 thrombosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In-stent restenosis , thrombosis , and aneurysm formation are known complications .
	manualset3
93473	3	399481	13	NULL	NULL	0	NULL	aneurysm formation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In-stent restenosis , thrombosis , and aneurysm formation are known complications .
	manualset3
93474	4	399481	13	NULL	NULL	0	NULL	complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In-stent restenosis , thrombosis , and aneurysm formation are known complications .
	manualset3
93475	1	399482	13	NULL	NULL	0	NULL	tiludronate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro , tiludronate added to bone tissue culture inhibits calcium release , lysosomal enzyme secretion and collagen matrix degradation when induced by various stimulators of bone resorption .
	manualset3
93476	2	399482	13	NULL	NULL	0	NULL	bone tissue culture	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro , tiludronate added to bone tissue culture inhibits calcium release , lysosomal enzyme secretion and collagen matrix degradation when induced by various stimulators of bone resorption .
	manualset3
93477	3	399482	13	NULL	NULL	0	NULL	calcium release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro , tiludronate added to bone tissue culture inhibits calcium release , lysosomal enzyme secretion and collagen matrix degradation when induced by various stimulators of bone resorption .
	manualset3
93478	4	399482	13	NULL	NULL	0	NULL	lysosomal enzyme secretion 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro , tiludronate added to bone tissue culture inhibits calcium release , lysosomal enzyme secretion and collagen matrix degradation when induced by various stimulators of bone resorption .
	manualset3
93479	5	399482	13	NULL	NULL	0	NULL	collagen matrix degradation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro , tiludronate added to bone tissue culture inhibits calcium release , lysosomal enzyme secretion and collagen matrix degradation when induced by various stimulators of bone resorption .
	manualset3
93480	6	399482	13	NULL	NULL	0	NULL	various stimulators	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro , tiludronate added to bone tissue culture inhibits calcium release , lysosomal enzyme secretion and collagen matrix degradation when induced by various stimulators of bone resorption .
	manualset3
93481	7	399482	13	NULL	NULL	0	NULL	bone resorption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro , tiludronate added to bone tissue culture inhibits calcium release , lysosomal enzyme secretion and collagen matrix degradation when induced by various stimulators of bone resorption .
	manualset3
93482	1	399483	13	NULL	NULL	0	NULL	effect 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro , we examined the effect of recombinant Ang-4 on endothelial cell migration in Boyden chambers .
	manualset3
93483	2	399483	13	NULL	NULL	0	NULL	recombinant Ang-4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro , we examined the effect of recombinant Ang-4 on endothelial cell migration in Boyden chambers .
	manualset3
93484	3	399483	13	NULL	NULL	0	NULL	endothelial cell migration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro , we examined the effect of recombinant Ang-4 on endothelial cell migration in Boyden chambers .
	manualset3
93485	4	399483	13	NULL	NULL	0	NULL	Boyden chambers	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro , we examined the effect of recombinant Ang-4 on endothelial cell migration in Boyden chambers .
	manualset3
93486	1	399484	13	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro activity of protegrin-1 and beta-defensin-1 , alone and in combination with isoniazid , against Mycobacterium tuberculosis .
	manualset3
93487	2	399484	13	NULL	NULL	0	NULL	protegrin-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro activity of protegrin-1 and beta-defensin-1 , alone and in combination with isoniazid , against Mycobacterium tuberculosis .
	manualset3
93488	3	399484	13	NULL	NULL	0	NULL	beta-defensin-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro activity of protegrin-1 and beta-defensin-1 , alone and in combination with isoniazid , against Mycobacterium tuberculosis .
	manualset3
93489	4	399484	13	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro activity of protegrin-1 and beta-defensin-1 , alone and in combination with isoniazid , against Mycobacterium tuberculosis .
	manualset3
93490	5	399484	13	NULL	NULL	0	NULL	isoniazid	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro activity of protegrin-1 and beta-defensin-1 , alone and in combination with isoniazid , against Mycobacterium tuberculosis .
	manualset3
93491	6	399484	13	NULL	NULL	0	NULL	Mycobacterium tuberculosis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro activity of protegrin-1 and beta-defensin-1 , alone and in combination with isoniazid , against Mycobacterium tuberculosis .
	manualset3
93492	1	399485	13	NULL	NULL	0	NULL	Thrombosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Thrombosis at the site of abdominal aortic aneurysm with repeated myocardial infarction ) .
	manualset3
93493	2	399485	13	NULL	NULL	0	NULL	site of abdominal aortic aneurysm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Thrombosis at the site of abdominal aortic aneurysm with repeated myocardial infarction ) .
	manualset3
93494	3	399485	13	NULL	NULL	0	NULL	myocardial infarction 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Thrombosis at the site of abdominal aortic aneurysm with repeated myocardial infarction ) .
	manualset3
93495	1	399486	13	NULL	NULL	0	NULL	 complementation experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro and in vivo complementation experiments revealed that at least five cistrons were concerned with head formation and that at least six cistrons were concerned with tail formation in phi80 .
	manualset3
93496	2	399486	13	NULL	NULL	0	NULL	five	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro and in vivo complementation experiments revealed that at least five cistrons were concerned with head formation and that at least six cistrons were concerned with tail formation in phi80 .
	manualset3
93497	3	399486	13	NULL	NULL	0	NULL	cistrons	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro and in vivo complementation experiments revealed that at least five cistrons were concerned with head formation and that at least six cistrons were concerned with tail formation in phi80 .
	manualset3
93498	4	399486	13	NULL	NULL	0	NULL	head formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro and in vivo complementation experiments revealed that at least five cistrons were concerned with head formation and that at least six cistrons were concerned with tail formation in phi80 .
	manualset3
93499	5	399486	13	NULL	NULL	0	NULL	six	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro and in vivo complementation experiments revealed that at least five cistrons were concerned with head formation and that at least six cistrons were concerned with tail formation in phi80 .
	manualset3
93500	6	399486	13	NULL	NULL	0	NULL	cistrons 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro and in vivo complementation experiments revealed that at least five cistrons were concerned with head formation and that at least six cistrons were concerned with tail formation in phi80 .
	manualset3
93501	7	399486	13	NULL	NULL	0	NULL	tail formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro and in vivo complementation experiments revealed that at least five cistrons were concerned with head formation and that at least six cistrons were concerned with tail formation in phi80 .
	manualset3
93502	8	399486	13	NULL	NULL	0	NULL	phi80 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro and in vivo complementation experiments revealed that at least five cistrons were concerned with head formation and that at least six cistrons were concerned with tail formation in phi80 .
	manualset3
93503	1	399487	13	NULL	NULL	0	NULL	In vitro studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro and in vivo studies of specific neuronal fast and slow transport components are presently reshaping our understanding of how the processes of vesicular and cytoskeletal transport are regulated in axons and dendrites .
	manualset3
93504	2	399487	13	NULL	NULL	0	NULL	in vivo studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro and in vivo studies of specific neuronal fast and slow transport components are presently reshaping our understanding of how the processes of vesicular and cytoskeletal transport are regulated in axons and dendrites .
	manualset3
93505	3	399487	13	NULL	NULL	0	NULL	specific neuronal fast 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro and in vivo studies of specific neuronal fast and slow transport components are presently reshaping our understanding of how the processes of vesicular and cytoskeletal transport are regulated in axons and dendrites .
	manualset3
93506	4	399487	13	NULL	NULL	0	NULL	transport components	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro and in vivo studies of specific neuronal fast and slow transport components are presently reshaping our understanding of how the processes of vesicular and cytoskeletal transport are regulated in axons and dendrites .
	manualset3
93507	5	399487	13	NULL	NULL	0	NULL	understanding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro and in vivo studies of specific neuronal fast and slow transport components are presently reshaping our understanding of how the processes of vesicular and cytoskeletal transport are regulated in axons and dendrites .
	manualset3
93508	6	399487	13	NULL	NULL	0	NULL	processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro and in vivo studies of specific neuronal fast and slow transport components are presently reshaping our understanding of how the processes of vesicular and cytoskeletal transport are regulated in axons and dendrites .
	manualset3
93509	7	399487	13	NULL	NULL	0	NULL	vesicular transport	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro and in vivo studies of specific neuronal fast and slow transport components are presently reshaping our understanding of how the processes of vesicular and cytoskeletal transport are regulated in axons and dendrites .
	manualset3
93510	8	399487	13	NULL	NULL	0	NULL	cytoskeletal transport	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro and in vivo studies of specific neuronal fast and slow transport components are presently reshaping our understanding of how the processes of vesicular and cytoskeletal transport are regulated in axons and dendrites .
	manualset3
93511	9	399487	13	NULL	NULL	0	NULL	axons	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro and in vivo studies of specific neuronal fast and slow transport components are presently reshaping our understanding of how the processes of vesicular and cytoskeletal transport are regulated in axons and dendrites .
	manualset3
93512	10	399487	13	NULL	NULL	0	NULL	dendrites	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro and in vivo studies of specific neuronal fast and slow transport components are presently reshaping our understanding of how the processes of vesicular and cytoskeletal transport are regulated in axons and dendrites .
	manualset3
93513	1	399488	13	NULL	NULL	0	NULL	In vitro suppression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro and in vivo suppression of growth of rat liver epithelial tumor cells by antisense oligonucleotide against protein kinase C-alpha .
	manualset3
93514	2	399488	13	NULL	NULL	0	NULL	in vivo suppression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro and in vivo suppression of growth of rat liver epithelial tumor cells by antisense oligonucleotide against protein kinase C-alpha .
	manualset3
93515	3	399488	13	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro and in vivo suppression of growth of rat liver epithelial tumor cells by antisense oligonucleotide against protein kinase C-alpha .
	manualset3
93516	4	399488	13	NULL	NULL	0	NULL	rat liver epithelial tumor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro and in vivo suppression of growth of rat liver epithelial tumor cells by antisense oligonucleotide against protein kinase C-alpha .
	manualset3
93517	5	399488	13	NULL	NULL	0	NULL	antisense oligonucleotide	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro and in vivo suppression of growth of rat liver epithelial tumor cells by antisense oligonucleotide against protein kinase C-alpha .
	manualset3
93518	6	399488	13	NULL	NULL	0	NULL	protein kinase C-alpha	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro and in vivo suppression of growth of rat liver epithelial tumor cells by antisense oligonucleotide against protein kinase C-alpha .
	manualset3
93519	1	399489	13	NULL	NULL	0	NULL	In vitro antifungal activities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro antifungal activities of bis ( alkylpyridinium ) alkane compounds against pathogenic yeasts and molds .
	manualset3
93520	2	399489	13	NULL	NULL	0	NULL	bis ( alkylpyridinium ) alkane compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro antifungal activities of bis ( alkylpyridinium ) alkane compounds against pathogenic yeasts and molds .
	manualset3
93521	3	399489	13	NULL	NULL	0	NULL	pathogenic yeasts	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro antifungal activities of bis ( alkylpyridinium ) alkane compounds against pathogenic yeasts and molds .
	manualset3
93522	4	399489	13	NULL	NULL	0	NULL	pathogenic molds	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro antifungal activities of bis ( alkylpyridinium ) alkane compounds against pathogenic yeasts and molds .
	manualset3
93523	1	399490	13	NULL	NULL	0	NULL	In vitro antimicrobial activities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro antimicrobial activities of the HPCS derivatives were evaluated by the Kirby-Bauer disc diffusion method and the macrotube dilution broth method .
	manualset3
93524	2	399490	13	NULL	NULL	0	NULL	HPCS derivatives 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro antimicrobial activities of the HPCS derivatives were evaluated by the Kirby-Bauer disc diffusion method and the macrotube dilution broth method .
	manualset3
93525	3	399490	13	NULL	NULL	0	NULL	Kirby-Bauer disc diffusion method	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro antimicrobial activities of the HPCS derivatives were evaluated by the Kirby-Bauer disc diffusion method and the macrotube dilution broth method .
	manualset3
93526	4	399490	13	NULL	NULL	0	NULL	macrotube dilution broth method	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro antimicrobial activities of the HPCS derivatives were evaluated by the Kirby-Bauer disc diffusion method and the macrotube dilution broth method .
	manualset3
93695	1	399491	13	NULL	NULL	0	NULL	In vitro antiviral activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro antiviral activity of mycophenolic acid and its reversal by guanine-type compounds .
	manualset3
93696	2	399491	13	NULL	NULL	0	NULL	mycophenolic acid	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro antiviral activity of mycophenolic acid and its reversal by guanine-type compounds .
	manualset3
93697	3	399491	13	NULL	NULL	0	NULL	reversal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro antiviral activity of mycophenolic acid and its reversal by guanine-type compounds .
	manualset3
93698	4	399491	13	NULL	NULL	0	NULL	 guanine-type compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro antiviral activity of mycophenolic acid and its reversal by guanine-type compounds .
	manualset3
93699	1	399492	13	NULL	NULL	0	NULL	In vitro assays 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro assays were used to assess non-2OG TCAIs as inhibitors of purified PHD2 and FIH .
	manualset3
93700	2	399492	13	NULL	NULL	0	NULL	non-2OG TCAIs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro assays were used to assess non-2OG TCAIs as inhibitors of purified PHD2 and FIH .
	manualset3
93701	3	399492	13	NULL	NULL	0	NULL	 inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro assays were used to assess non-2OG TCAIs as inhibitors of purified PHD2 and FIH .
	manualset3
93702	4	399492	13	NULL	NULL	0	NULL	PHD2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro assays were used to assess non-2OG TCAIs as inhibitors of purified PHD2 and FIH .
	manualset3
93703	5	399492	13	NULL	NULL	0	NULL	FIH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro assays were used to assess non-2OG TCAIs as inhibitors of purified PHD2 and FIH .
	manualset3
93704	1	399493	13	NULL	NULL	0	NULL	In vitro effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro effect of immune complex positive human sera on antibody dependent cellular cytotoxicity .
	manualset3
93705	2	399493	13	NULL	NULL	0	NULL	 immune complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro effect of immune complex positive human sera on antibody dependent cellular cytotoxicity .
	manualset3
93706	3	399493	13	NULL	NULL	0	NULL	human sera	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro effect of immune complex positive human sera on antibody dependent cellular cytotoxicity .
	manualset3
93707	4	399493	13	NULL	NULL	0	NULL	 antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro effect of immune complex positive human sera on antibody dependent cellular cytotoxicity .
	manualset3
93708	5	399493	13	NULL	NULL	0	NULL	cellular cytotoxicity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro effect of immune complex positive human sera on antibody dependent cellular cytotoxicity .
	manualset3
93709	1	399494	13	NULL	NULL	0	NULL	Thrombotic changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Thrombotic changes in hemostasis following streptokinase therapy in myocardial infarct ) .
	manualset3
93710	2	399494	13	NULL	NULL	0	NULL	hemostasis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Thrombotic changes in hemostasis following streptokinase therapy in myocardial infarct ) .
	manualset3
93711	3	399494	13	NULL	NULL	0	NULL	streptokinase therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Thrombotic changes in hemostasis following streptokinase therapy in myocardial infarct ) .
	manualset3
93712	4	399494	13	NULL	NULL	0	NULL	myocardial infarct	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Thrombotic changes in hemostasis following streptokinase therapy in myocardial infarct ) .
	manualset3
93713	1	399495	13	NULL	NULL	NULL	NULL	In vitro effects	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In vitro effects of R-verapamil on the cytokine environment and T-lymphocyte proliferation when human T-lymphocyte activation takes place in the presence of acute myelogenous leukemia blasts .
	manualset3
93714	2	399495	13	NULL	NULL	0	NULL	 R-verapamil	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro effects of R-verapamil on the cytokine environment and T-lymphocyte proliferation when human T-lymphocyte activation takes place in the presence of acute myelogenous leukemia blasts .
	manualset3
93715	3	399495	13	NULL	NULL	0	NULL	cytokine environment	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro effects of R-verapamil on the cytokine environment and T-lymphocyte proliferation when human T-lymphocyte activation takes place in the presence of acute myelogenous leukemia blasts .
	manualset3
93716	4	399495	13	NULL	NULL	0	NULL	T-lymphocyte proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro effects of R-verapamil on the cytokine environment and T-lymphocyte proliferation when human T-lymphocyte activation takes place in the presence of acute myelogenous leukemia blasts .
	manualset3
93717	5	399495	13	NULL	NULL	0	NULL	 human T-lymphocyte activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro effects of R-verapamil on the cytokine environment and T-lymphocyte proliferation when human T-lymphocyte activation takes place in the presence of acute myelogenous leukemia blasts .
	manualset3
93718	6	399495	13	NULL	NULL	0	NULL	presence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro effects of R-verapamil on the cytokine environment and T-lymphocyte proliferation when human T-lymphocyte activation takes place in the presence of acute myelogenous leukemia blasts .
	manualset3
93719	7	399495	13	NULL	NULL	0	NULL	acute myelogenous leukemia blasts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro effects of R-verapamil on the cytokine environment and T-lymphocyte proliferation when human T-lymphocyte activation takes place in the presence of acute myelogenous leukemia blasts .
	manualset3
93720	1	399496	13	NULL	NULL	0	NULL	In vitro experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro experiments using alkaline phosphatase and osteocalcin assays demonstrated the proliferation and differentiation of MSC into osteoblast-like cells , especially the direct contact between VEC and MSC .
	manualset3
93721	2	399496	13	NULL	NULL	0	NULL	alkaline phosphatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro experiments using alkaline phosphatase and osteocalcin assays demonstrated the proliferation and differentiation of MSC into osteoblast-like cells , especially the direct contact between VEC and MSC .
	manualset3
93722	3	399496	13	NULL	NULL	0	NULL	osteocalcin assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro experiments using alkaline phosphatase and osteocalcin assays demonstrated the proliferation and differentiation of MSC into osteoblast-like cells , especially the direct contact between VEC and MSC .
	manualset3
93723	4	399496	13	NULL	NULL	0	NULL	proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro experiments using alkaline phosphatase and osteocalcin assays demonstrated the proliferation and differentiation of MSC into osteoblast-like cells , especially the direct contact between VEC and MSC .
	manualset3
93724	5	399496	13	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro experiments using alkaline phosphatase and osteocalcin assays demonstrated the proliferation and differentiation of MSC into osteoblast-like cells , especially the direct contact between VEC and MSC .
	manualset3
93725	6	399496	13	NULL	NULL	0	NULL	MSC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro experiments using alkaline phosphatase and osteocalcin assays demonstrated the proliferation and differentiation of MSC into osteoblast-like cells , especially the direct contact between VEC and MSC .
	manualset3
93726	7	399496	13	NULL	NULL	0	NULL	osteoblast-like cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro experiments using alkaline phosphatase and osteocalcin assays demonstrated the proliferation and differentiation of MSC into osteoblast-like cells , especially the direct contact between VEC and MSC .
	manualset3
93727	8	399496	13	NULL	NULL	0	NULL	contact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro experiments using alkaline phosphatase and osteocalcin assays demonstrated the proliferation and differentiation of MSC into osteoblast-like cells , especially the direct contact between VEC and MSC .
	manualset3
93728	9	399496	13	NULL	NULL	0	NULL	VEC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro experiments using alkaline phosphatase and osteocalcin assays demonstrated the proliferation and differentiation of MSC into osteoblast-like cells , especially the direct contact between VEC and MSC .
	manualset3
93729	10	399496	13	NULL	NULL	0	NULL	MSC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro experiments using alkaline phosphatase and osteocalcin assays demonstrated the proliferation and differentiation of MSC into osteoblast-like cells , especially the direct contact between VEC and MSC .
	manualset3
93730	1	399497	13	NULL	NULL	0	NULL	In vitro growth of colonies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro growth of colonies of mitogen-stimulated mouse T lymphocytes : I. Conditions affecting colony formation ; II .
	manualset3
93731	2	399497	13	NULL	NULL	0	NULL	mitogen-stimulated mouse T lymphocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro growth of colonies of mitogen-stimulated mouse T lymphocytes : I. Conditions affecting colony formation ; II .
	manualset3
93732	3	399497	13	NULL	NULL	0	NULL	Conditions 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro growth of colonies of mitogen-stimulated mouse T lymphocytes : I. Conditions affecting colony formation ; II .
	manualset3
93733	4	399497	13	NULL	NULL	0	NULL	colony formation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro growth of colonies of mitogen-stimulated mouse T lymphocytes : I. Conditions affecting colony formation ; II .
	manualset3
93734	1	399498	13	NULL	NULL	0	NULL	In vitro kinetic studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro kinetic studies revealed that these compounds are among the most effective APN/CD13 inhibitors found so far .
	manualset3
93735	2	399498	13	NULL	NULL	0	NULL	compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro kinetic studies revealed that these compounds are among the most effective APN/CD13 inhibitors found so far .
	manualset3
93736	3	399498	13	NULL	NULL	0	NULL	effective APN/CD13 inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro kinetic studies revealed that these compounds are among the most effective APN/CD13 inhibitors found so far .
	manualset3
93737	1	399499	13	NULL	NULL	0	NULL	In vitro lymphoma cell growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro lymphoma cell growth could be maintained in the presence of the growth factor for up to five weeks .
	manualset3
93738	2	399499	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro lymphoma cell growth could be maintained in the presence of the growth factor for up to five weeks .
	manualset3
93739	3	399499	13	NULL	NULL	0	NULL	growth factor	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro lymphoma cell growth could be maintained in the presence of the growth factor for up to five weeks .
	manualset3
93740	4	399499	13	NULL	NULL	0	NULL	five weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro lymphoma cell growth could be maintained in the presence of the growth factor for up to five weeks .
	manualset3
93741	1	399500	13	NULL	NULL	0	NULL	In vitro pharmacological purging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro pharmacological purging of human bone marrow is enhanced by the use of lonidamine .
	manualset3
93742	2	399500	13	NULL	NULL	0	NULL	human bone marrow	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro pharmacological purging of human bone marrow is enhanced by the use of lonidamine .
	manualset3
93743	3	399500	13	NULL	NULL	NULL	NULL	use	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In vitro pharmacological purging of human bone marrow is enhanced by the use of lonidamine .
	manualset3
93744	4	399500	13	NULL	NULL	0	NULL	lonidamine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro pharmacological purging of human bone marrow is enhanced by the use of lonidamine .
	manualset3
93745	1	399501	13	NULL	NULL	0	NULL	In vitro protein binding studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro protein binding studies suggest that AP-1 complexes are capable of binding to PE2A .
	manualset3
93746	2	399501	13	NULL	NULL	0	NULL	AP-1 complexes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro protein binding studies suggest that AP-1 complexes are capable of binding to PE2A .
	manualset3
93747	4	399501	13	NULL	NULL	NULL	NULL	PE2A	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In vitro protein binding studies suggest that AP-1 complexes are capable of binding to PE2A .
	manualset3
93748	3	399501	13	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro protein binding studies suggest that AP-1 complexes are capable of binding to PE2A .
	manualset3
93749	1	399502	13	NULL	NULL	0	NULL	In vitro selection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro selection of NIH-3T3 cells for resistance to lymphotoxin induces resistance to activated macrophages and enhances tumorigenicity in vivo .
	manualset3
93750	2	399502	13	NULL	NULL	0	NULL	NIH-3T3 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro selection of NIH-3T3 cells for resistance to lymphotoxin induces resistance to activated macrophages and enhances tumorigenicity in vivo .
	manualset3
93751	3	399502	13	NULL	NULL	0	NULL	resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro selection of NIH-3T3 cells for resistance to lymphotoxin induces resistance to activated macrophages and enhances tumorigenicity in vivo .
	manualset3
93752	4	399502	13	NULL	NULL	0	NULL	lymphotoxin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro selection of NIH-3T3 cells for resistance to lymphotoxin induces resistance to activated macrophages and enhances tumorigenicity in vivo .
	manualset3
93753	5	399502	13	NULL	NULL	0	NULL	resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro selection of NIH-3T3 cells for resistance to lymphotoxin induces resistance to activated macrophages and enhances tumorigenicity in vivo .
	manualset3
93754	6	399502	13	NULL	NULL	0	NULL	macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro selection of NIH-3T3 cells for resistance to lymphotoxin induces resistance to activated macrophages and enhances tumorigenicity in vivo .
	manualset3
93755	7	399502	13	NULL	NULL	0	NULL	tumorigenicity in vivo 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro selection of NIH-3T3 cells for resistance to lymphotoxin induces resistance to activated macrophages and enhances tumorigenicity in vivo .
	manualset3
93756	1	399503	13	NULL	NULL	0	NULL	In vitro studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro studies of cell division have revealed similar mechanisms .
	manualset3
93757	2	399503	13	NULL	NULL	0	NULL	cell division	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro studies of cell division have revealed similar mechanisms .
	manualset3
93758	3	399503	13	NULL	NULL	0	NULL	similar mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro studies of cell division have revealed similar mechanisms .
	manualset3
93759	1	399504	13	NULL	NULL	0	NULL	In vitro studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro studies of human breast carcinoma cells obtained by aspiration biopsy .
	manualset3
93760	2	399504	13	NULL	NULL	0	NULL	human breast carcinoma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro studies of human breast carcinoma cells obtained by aspiration biopsy .
	manualset3
93761	3	399504	13	NULL	NULL	0	NULL	aspiration biopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro studies of human breast carcinoma cells obtained by aspiration biopsy .
	manualset3
93762	1	399505	13	NULL	NULL	0	NULL	In vitro studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro studies with crude membranes isolated from recombinant strains revealed that BRUCELLA : cyclic 1 , 2-beta-glucan synthetase was not inhibited by high concentrations of KCl or potassium glutamate even when expressed in AGROBACTERIUM : or RHIZOBIUM : backgrounds .
	manualset3
93763	2	399505	13	NULL	NULL	0	NULL	crude membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro studies with crude membranes isolated from recombinant strains revealed that BRUCELLA : cyclic 1 , 2-beta-glucan synthetase was not inhibited by high concentrations of KCl or potassium glutamate even when expressed in AGROBACTERIUM : or RHIZOBIUM : backgrounds .
	manualset3
93764	3	399505	13	NULL	NULL	0	NULL	recombinant strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro studies with crude membranes isolated from recombinant strains revealed that BRUCELLA : cyclic 1 , 2-beta-glucan synthetase was not inhibited by high concentrations of KCl or potassium glutamate even when expressed in AGROBACTERIUM : or RHIZOBIUM : backgrounds .
	manualset3
93765	4	399505	13	NULL	NULL	0	NULL	 BRUCELLA	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro studies with crude membranes isolated from recombinant strains revealed that BRUCELLA : cyclic 1 , 2-beta-glucan synthetase was not inhibited by high concentrations of KCl or potassium glutamate even when expressed in AGROBACTERIUM : or RHIZOBIUM : backgrounds .
	manualset3
93766	5	399505	13	NULL	NULL	0	NULL	cyclic 1 , 2-beta-glucan synthetase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro studies with crude membranes isolated from recombinant strains revealed that BRUCELLA : cyclic 1 , 2-beta-glucan synthetase was not inhibited by high concentrations of KCl or potassium glutamate even when expressed in AGROBACTERIUM : or RHIZOBIUM : backgrounds .
	manualset3
93767	6	399505	13	NULL	NULL	0	NULL	high concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro studies with crude membranes isolated from recombinant strains revealed that BRUCELLA : cyclic 1 , 2-beta-glucan synthetase was not inhibited by high concentrations of KCl or potassium glutamate even when expressed in AGROBACTERIUM : or RHIZOBIUM : backgrounds .
	manualset3
93768	7	399505	13	NULL	NULL	0	NULL	KCl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro studies with crude membranes isolated from recombinant strains revealed that BRUCELLA : cyclic 1 , 2-beta-glucan synthetase was not inhibited by high concentrations of KCl or potassium glutamate even when expressed in AGROBACTERIUM : or RHIZOBIUM : backgrounds .
	manualset3
93769	8	399505	13	NULL	NULL	0	NULL	potassium glutamate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro studies with crude membranes isolated from recombinant strains revealed that BRUCELLA : cyclic 1 , 2-beta-glucan synthetase was not inhibited by high concentrations of KCl or potassium glutamate even when expressed in AGROBACTERIUM : or RHIZOBIUM : backgrounds .
	manualset3
93770	9	399505	13	NULL	NULL	0	NULL	AGROBACTERIUM	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro studies with crude membranes isolated from recombinant strains revealed that BRUCELLA : cyclic 1 , 2-beta-glucan synthetase was not inhibited by high concentrations of KCl or potassium glutamate even when expressed in AGROBACTERIUM : or RHIZOBIUM : backgrounds .
	manualset3
93771	10	399505	13	NULL	NULL	0	NULL	RHIZOBIUM	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro studies with crude membranes isolated from recombinant strains revealed that BRUCELLA : cyclic 1 , 2-beta-glucan synthetase was not inhibited by high concentrations of KCl or potassium glutamate even when expressed in AGROBACTERIUM : or RHIZOBIUM : backgrounds .
	manualset3
93772	1	399506	13	NULL	NULL	0	NULL	In vitro tissue chambers	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro tissue chambers , like those used for electrophysiology , are usually continually perfused with the gassed buffer , but stopping the perfusion to add expensive chemicals or acquire imaging data is a common practice .
	manualset3
93773	2	399506	13	NULL	NULL	0	NULL	electrophysiology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro tissue chambers , like those used for electrophysiology , are usually continually perfused with the gassed buffer , but stopping the perfusion to add expensive chemicals or acquire imaging data is a common practice .
	manualset3
93774	3	399506	13	NULL	NULL	0	NULL	gassed buffer	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro tissue chambers , like those used for electrophysiology , are usually continually perfused with the gassed buffer , but stopping the perfusion to add expensive chemicals or acquire imaging data is a common practice .
	manualset3
93775	4	399506	13	NULL	NULL	0	NULL	perfusion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro tissue chambers , like those used for electrophysiology , are usually continually perfused with the gassed buffer , but stopping the perfusion to add expensive chemicals or acquire imaging data is a common practice .
	manualset3
93776	5	399506	13	NULL	NULL	0	NULL	expensive chemicals 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro tissue chambers , like those used for electrophysiology , are usually continually perfused with the gassed buffer , but stopping the perfusion to add expensive chemicals or acquire imaging data is a common practice .
	manualset3
93777	6	399506	13	NULL	NULL	0	NULL	imaging data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro tissue chambers , like those used for electrophysiology , are usually continually perfused with the gassed buffer , but stopping the perfusion to add expensive chemicals or acquire imaging data is a common practice .
	manualset3
93778	7	399506	13	NULL	NULL	0	NULL	common practice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro tissue chambers , like those used for electrophysiology , are usually continually perfused with the gassed buffer , but stopping the perfusion to add expensive chemicals or acquire imaging data is a common practice .
	manualset3
93779	1	399507	13	NULL	NULL	0	NULL	In vitro translation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro translation directed by mRNA isolated from these cells has shown that the primary translation products are preprobactenecins of 23.5 and 21 kD , and are processed to polypeptides of 20 and 15.8 kD , respectively .
	manualset3
93780	2	399507	13	NULL	NULL	0	NULL	mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro translation directed by mRNA isolated from these cells has shown that the primary translation products are preprobactenecins of 23.5 and 21 kD , and are processed to polypeptides of 20 and 15.8 kD , respectively .
	manualset3
93781	3	399507	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro translation directed by mRNA isolated from these cells has shown that the primary translation products are preprobactenecins of 23.5 and 21 kD , and are processed to polypeptides of 20 and 15.8 kD , respectively .
	manualset3
93782	4	399507	13	NULL	NULL	0	NULL	primary translation products	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro translation directed by mRNA isolated from these cells has shown that the primary translation products are preprobactenecins of 23.5 and 21 kD , and are processed to polypeptides of 20 and 15.8 kD , respectively .
	manualset3
93783	5	399507	13	NULL	NULL	0	NULL	 preprobactenecins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro translation directed by mRNA isolated from these cells has shown that the primary translation products are preprobactenecins of 23.5 and 21 kD , and are processed to polypeptides of 20 and 15.8 kD , respectively .
	manualset3
93784	6	399507	13	NULL	NULL	0	NULL	23.5 kD	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro translation directed by mRNA isolated from these cells has shown that the primary translation products are preprobactenecins of 23.5 and 21 kD , and are processed to polypeptides of 20 and 15.8 kD , respectively .
	manualset3
93785	7	399507	13	NULL	NULL	0	NULL	21 kD	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro translation directed by mRNA isolated from these cells has shown that the primary translation products are preprobactenecins of 23.5 and 21 kD , and are processed to polypeptides of 20 and 15.8 kD , respectively .
	manualset3
93786	8	399507	13	NULL	NULL	NULL	NULL	polypeptides of 20 kD	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In vitro translation directed by mRNA isolated from these cells has shown that the primary translation products are preprobactenecins of 23.5 and 21 kD , and are processed to polypeptides of 20 and 15.8 kD , respectively .
	manualset3
93787	9	399507	13	NULL	NULL	0	NULL	polypeptides of 15.8 kD	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro translation directed by mRNA isolated from these cells has shown that the primary translation products are preprobactenecins of 23.5 and 21 kD , and are processed to polypeptides of 20 and 15.8 kD , respectively .
	manualset3
93788	1	399508	13	NULL	NULL	0	NULL	In vitro ubiquitination assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro ubiquitination assay showed that SCFbeta-TrCP but not SCFFBW4 increased ubiquitination of RCAN1 , dependent on H2O2 stimulation .
	manualset3
93789	2	399508	13	NULL	NULL	0	NULL	SCFbeta-TrCP	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro ubiquitination assay showed that SCFbeta-TrCP but not SCFFBW4 increased ubiquitination of RCAN1 , dependent on H2O2 stimulation .
	manualset3
93790	3	399508	13	NULL	NULL	0	NULL	SCFFBW4	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro ubiquitination assay showed that SCFbeta-TrCP but not SCFFBW4 increased ubiquitination of RCAN1 , dependent on H2O2 stimulation .
	manualset3
93791	4	399508	13	NULL	NULL	0	NULL	ubiquitination 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro ubiquitination assay showed that SCFbeta-TrCP but not SCFFBW4 increased ubiquitination of RCAN1 , dependent on H2O2 stimulation .
	manualset3
93792	5	399508	13	NULL	NULL	0	NULL	RCAN1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro ubiquitination assay showed that SCFbeta-TrCP but not SCFFBW4 increased ubiquitination of RCAN1 , dependent on H2O2 stimulation .
	manualset3
93793	6	399508	13	NULL	NULL	0	NULL	H2O2 stimulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro ubiquitination assay showed that SCFbeta-TrCP but not SCFFBW4 increased ubiquitination of RCAN1 , dependent on H2O2 stimulation .
	manualset3
93794	1	399509	13	NULL	NULL	0	NULL	In vitro vs. in vivo tape stripping 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro vs. in vivo tape stripping : Validation of the porcine ear model and penetration assessment of novel sucrose stearate emulsions .
	manualset3
93795	2	399509	13	NULL	NULL	0	NULL	Validation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro vs. in vivo tape stripping : Validation of the porcine ear model and penetration assessment of novel sucrose stearate emulsions .
	manualset3
93796	3	399509	13	NULL	NULL	NULL	NULL	porcine ear model 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In vitro vs. in vivo tape stripping : Validation of the porcine ear model and penetration assessment of novel sucrose stearate emulsions .
	manualset3
93797	4	399509	13	NULL	NULL	0	NULL	penetration assessment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro vs. in vivo tape stripping : Validation of the porcine ear model and penetration assessment of novel sucrose stearate emulsions .
	manualset3
93798	5	399509	13	NULL	NULL	0	NULL	novel sucrose stearate emulsions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro vs. in vivo tape stripping : Validation of the porcine ear model and penetration assessment of novel sucrose stearate emulsions .
	manualset3
93799	1	399510	13	NULL	NULL	0	NULL	higher expression levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro we observed higher expression levels and sustained long-term expression of TK .007 , indicating lower nonspecific toxicity .
	manualset3
93800	2	399510	13	NULL	NULL	0	NULL	expression of TK .007	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro we observed higher expression levels and sustained long-term expression of TK .007 , indicating lower nonspecific toxicity .
	manualset3
93801	3	399510	13	NULL	NULL	0	NULL	lower nonspecific toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro we observed higher expression levels and sustained long-term expression of TK .007 , indicating lower nonspecific toxicity .
	manualset3
93802	1	399511	13	NULL	NULL	NULL	NULL	10 min	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In vivo , 10 min of umbilical cord occlusion produced an increase in fetal blood ionized magnesium concentration in all animals ( P = 0.02 ) that was temporally related to the decrease in fetal blood pH. .
	manualset3
93803	2	399511	13	NULL	NULL	0	NULL	umbilical cord occlusion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo , 10 min of umbilical cord occlusion produced an increase in fetal blood ionized magnesium concentration in all animals ( P = 0.02 ) that was temporally related to the decrease in fetal blood pH. .
	manualset3
93804	3	399511	13	NULL	NULL	NULL	NULL	increase in fetal blood ionized magnesium concentration	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In vivo , 10 min of umbilical cord occlusion produced an increase in fetal blood ionized magnesium concentration in all animals ( P = 0.02 ) that was temporally related to the decrease in fetal blood pH. .
	manualset3
93805	4	399511	13	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo , 10 min of umbilical cord occlusion produced an increase in fetal blood ionized magnesium concentration in all animals ( P = 0.02 ) that was temporally related to the decrease in fetal blood pH. .
	manualset3
93806	5	399511	13	NULL	NULL	0	NULL	P = 0.02	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo , 10 min of umbilical cord occlusion produced an increase in fetal blood ionized magnesium concentration in all animals ( P = 0.02 ) that was temporally related to the decrease in fetal blood pH. .
	manualset3
93807	6	399511	13	NULL	NULL	0	NULL	decrease in fetal blood pH	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo , 10 min of umbilical cord occlusion produced an increase in fetal blood ionized magnesium concentration in all animals ( P = 0.02 ) that was temporally related to the decrease in fetal blood pH. .
	manualset3
93808	1	399512	13	NULL	NULL	0	NULL	In vivo studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo , ex-vivo , and in vitro studies showed that TFF1 expression suppressed TNF -- mediated NF-B activation through the TNF receptor 1 ( TNFR1 ) / IB kinase ( IKK ) pathway .
	manualset3
93809	2	399512	13	NULL	NULL	0	NULL	ex-vivo studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo , ex-vivo , and in vitro studies showed that TFF1 expression suppressed TNF -- mediated NF-B activation through the TNF receptor 1 ( TNFR1 ) / IB kinase ( IKK ) pathway .
	manualset3
93810	3	399512	13	NULL	NULL	0	NULL	in vitro studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo , ex-vivo , and in vitro studies showed that TFF1 expression suppressed TNF -- mediated NF-B activation through the TNF receptor 1 ( TNFR1 ) / IB kinase ( IKK ) pathway .
	manualset3
93811	4	399512	13	NULL	NULL	0	NULL	TFF1 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo , ex-vivo , and in vitro studies showed that TFF1 expression suppressed TNF -- mediated NF-B activation through the TNF receptor 1 ( TNFR1 ) / IB kinase ( IKK ) pathway .
	manualset3
93812	5	399512	13	NULL	NULL	0	NULL	TNF -- mediated NF-B activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo , ex-vivo , and in vitro studies showed that TFF1 expression suppressed TNF -- mediated NF-B activation through the TNF receptor 1 ( TNFR1 ) / IB kinase ( IKK ) pathway .
	manualset3
93813	6	399512	13	NULL	NULL	0	NULL	TNF receptor 1 ( TNFR1 ) / IB kinase ( IKK ) pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo , ex-vivo , and in vitro studies showed that TFF1 expression suppressed TNF -- mediated NF-B activation through the TNF receptor 1 ( TNFR1 ) / IB kinase ( IKK ) pathway .
	manualset3
93814	1	399513	13	NULL	NULL	0	NULL	enzyme 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo , the enzyme but not the KOH solution produced shortening of p-aramid but not cellulose RFP recovered from the lungs .
	manualset3
93815	2	399513	13	NULL	NULL	0	NULL	 KOH solution 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo , the enzyme but not the KOH solution produced shortening of p-aramid but not cellulose RFP recovered from the lungs .
	manualset3
93816	3	399513	13	NULL	NULL	NULL	NULL	shortening of p-aramid 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In vivo , the enzyme but not the KOH solution produced shortening of p-aramid but not cellulose RFP recovered from the lungs .
	manualset3
93817	4	399513	13	NULL	NULL	0	NULL	shortening of cellulose RFP	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo , the enzyme but not the KOH solution produced shortening of p-aramid but not cellulose RFP recovered from the lungs .
	manualset3
93818	5	399513	13	NULL	NULL	0	NULL	lungs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo , the enzyme but not the KOH solution produced shortening of p-aramid but not cellulose RFP recovered from the lungs .
	manualset3
93819	1	399514	13	NULL	NULL	0	NULL	Tissue-phantom-dose relationship R ( t , F )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( Tissue-phantom-dose relationship R ( t , F ) for irradiation planning .
	manualset3
93820	2	399514	13	NULL	NULL	0	NULL	irradiation planning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Tissue-phantom-dose relationship R ( t , F ) for irradiation planning .
	manualset3
93821	1	399515	13	NULL	NULL	0	NULL	tumor growth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo , tumor growth was significantly reduced and overall survival significantly prolonged in mice treated with EA as compared to untreated mice .
	manualset3
93822	2	399515	13	NULL	NULL	0	NULL	overall survival 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo , tumor growth was significantly reduced and overall survival significantly prolonged in mice treated with EA as compared to untreated mice .
	manualset3
93823	3	399515	13	NULL	NULL	0	NULL	mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo , tumor growth was significantly reduced and overall survival significantly prolonged in mice treated with EA as compared to untreated mice .
	manualset3
93824	4	399515	13	NULL	NULL	0	NULL	EA	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo , tumor growth was significantly reduced and overall survival significantly prolonged in mice treated with EA as compared to untreated mice .
	manualset3
93825	5	399515	13	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo , tumor growth was significantly reduced and overall survival significantly prolonged in mice treated with EA as compared to untreated mice .
	manualset3
93826	1	399516	13	NULL	NULL	0	NULL	In vivo administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo administration of anti-CD4 monoclonal antibody prolongs survival in longtailed macaques with experimental allergic encephalomyelitis .
	manualset3
93827	2	399516	13	NULL	NULL	0	NULL	 anti-CD4 monoclonal antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo administration of anti-CD4 monoclonal antibody prolongs survival in longtailed macaques with experimental allergic encephalomyelitis .
	manualset3
93828	3	399516	13	NULL	NULL	0	NULL	survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo administration of anti-CD4 monoclonal antibody prolongs survival in longtailed macaques with experimental allergic encephalomyelitis .
	manualset3
93829	4	399516	13	NULL	NULL	0	NULL	longtailed macaques	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo administration of anti-CD4 monoclonal antibody prolongs survival in longtailed macaques with experimental allergic encephalomyelitis .
	manualset3
93830	5	399516	13	NULL	NULL	0	NULL	experimental allergic encephalomyelitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo administration of anti-CD4 monoclonal antibody prolongs survival in longtailed macaques with experimental allergic encephalomyelitis .
	manualset3
93831	1	399517	13	NULL	NULL	0	NULL	In vivo assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo assay showed that gut trypsin activity from L ( 4 ) treated with M. oleifera flower extract decreased over time ( 0-1 , 440 min ) and was strongly inhibited ( 98.6 % ) after 310 min incubation ; acetylcholinesterase activity was not affected .
	manualset3
93832	2	399517	13	NULL	NULL	NULL	NULL	gut trypsin activity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In vivo assay showed that gut trypsin activity from L ( 4 ) treated with M. oleifera flower extract decreased over time ( 0-1 , 440 min ) and was strongly inhibited ( 98.6 % ) after 310 min incubation ; acetylcholinesterase activity was not affected .
	manualset3
93833	3	399517	13	NULL	NULL	NULL	NULL	L ( 4 ) 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In vivo assay showed that gut trypsin activity from L ( 4 ) treated with M. oleifera flower extract decreased over time ( 0-1 , 440 min ) and was strongly inhibited ( 98.6 % ) after 310 min incubation ; acetylcholinesterase activity was not affected .
	manualset3
93834	4	399517	13	NULL	NULL	0	NULL	M. oleifera flower extract	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo assay showed that gut trypsin activity from L ( 4 ) treated with M. oleifera flower extract decreased over time ( 0-1 , 440 min ) and was strongly inhibited ( 98.6 % ) after 310 min incubation ; acetylcholinesterase activity was not affected .
	manualset3
93835	5	399517	13	NULL	NULL	0	NULL	time ( 0-1 , 440 min ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo assay showed that gut trypsin activity from L ( 4 ) treated with M. oleifera flower extract decreased over time ( 0-1 , 440 min ) and was strongly inhibited ( 98.6 % ) after 310 min incubation ; acetylcholinesterase activity was not affected .
	manualset3
93836	6	399517	13	NULL	NULL	0	NULL	98.6 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo assay showed that gut trypsin activity from L ( 4 ) treated with M. oleifera flower extract decreased over time ( 0-1 , 440 min ) and was strongly inhibited ( 98.6 % ) after 310 min incubation ; acetylcholinesterase activity was not affected .
	manualset3
93837	7	399517	13	NULL	NULL	NULL	NULL	310 min	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In vivo assay showed that gut trypsin activity from L ( 4 ) treated with M. oleifera flower extract decreased over time ( 0-1 , 440 min ) and was strongly inhibited ( 98.6 % ) after 310 min incubation ; acetylcholinesterase activity was not affected .
	manualset3
93838	8	399517	13	NULL	NULL	0	NULL	incubation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo assay showed that gut trypsin activity from L ( 4 ) treated with M. oleifera flower extract decreased over time ( 0-1 , 440 min ) and was strongly inhibited ( 98.6 % ) after 310 min incubation ; acetylcholinesterase activity was not affected .
	manualset3
93839	9	399517	13	NULL	NULL	0	NULL	acetylcholinesterase activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo assay showed that gut trypsin activity from L ( 4 ) treated with M. oleifera flower extract decreased over time ( 0-1 , 440 min ) and was strongly inhibited ( 98.6 % ) after 310 min incubation ; acetylcholinesterase activity was not affected .
	manualset3
93840	1	399518	13	NULL	NULL	0	NULL	In vivo competition experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo competition experiments confirmed that the enhanced detection capability of EPTA-Gd was based specifically on ER targeting .
	manualset3
93841	2	399518	13	NULL	NULL	0	NULL	detection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo competition experiments confirmed that the enhanced detection capability of EPTA-Gd was based specifically on ER targeting .
	manualset3
93842	3	399518	13	NULL	NULL	0	NULL	EPTA-Gd 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo competition experiments confirmed that the enhanced detection capability of EPTA-Gd was based specifically on ER targeting .
	manualset3
93843	4	399518	13	NULL	NULL	0	NULL	ER targeting 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo competition experiments confirmed that the enhanced detection capability of EPTA-Gd was based specifically on ER targeting .
	manualset3
93844	1	399519	13	NULL	NULL	0	NULL	In vivo depletion experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo depletion experiments show that CD4 + T cells are required for the SEB-triggered shock , while CD8 + cells suppress it .
	manualset3
93845	2	399519	13	NULL	NULL	0	NULL	CD4 + T cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo depletion experiments show that CD4 + T cells are required for the SEB-triggered shock , while CD8 + cells suppress it .
	manualset3
93846	3	399519	13	NULL	NULL	0	NULL	SEB-triggered shock	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo depletion experiments show that CD4 + T cells are required for the SEB-triggered shock , while CD8 + cells suppress it .
	manualset3
93847	4	399519	13	NULL	NULL	0	NULL	CD8 + cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo depletion experiments show that CD4 + T cells are required for the SEB-triggered shock , while CD8 + cells suppress it .
	manualset3
93848	1	399520	13	NULL	NULL	0	NULL	In vivo evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo evidence for stimulation of placental , myometrial , and endometrial prostaglandin G/H synthase 2 by fetal cortisol replacement after fetal adrenalectomy .
	manualset3
93849	2	399520	13	NULL	NULL	0	NULL	stimulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo evidence for stimulation of placental , myometrial , and endometrial prostaglandin G/H synthase 2 by fetal cortisol replacement after fetal adrenalectomy .
	manualset3
93850	3	399520	13	NULL	NULL	0	NULL	placental prostaglandin G/H synthase 2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo evidence for stimulation of placental , myometrial , and endometrial prostaglandin G/H synthase 2 by fetal cortisol replacement after fetal adrenalectomy .
	manualset3
93851	4	399520	13	NULL	NULL	0	NULL	myometrial prostaglandin G/H synthase 2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo evidence for stimulation of placental , myometrial , and endometrial prostaglandin G/H synthase 2 by fetal cortisol replacement after fetal adrenalectomy .
	manualset3
93852	5	399520	13	NULL	NULL	0	NULL	endometrial prostaglandin G/H synthase 2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo evidence for stimulation of placental , myometrial , and endometrial prostaglandin G/H synthase 2 by fetal cortisol replacement after fetal adrenalectomy .
	manualset3
93853	6	399520	13	NULL	NULL	0	NULL	fetal cortisol replacement	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo evidence for stimulation of placental , myometrial , and endometrial prostaglandin G/H synthase 2 by fetal cortisol replacement after fetal adrenalectomy .
	manualset3
93854	7	399520	13	NULL	NULL	0	NULL	 fetal adrenalectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo evidence for stimulation of placental , myometrial , and endometrial prostaglandin G/H synthase 2 by fetal cortisol replacement after fetal adrenalectomy .
	manualset3
94035	1	399521	13	NULL	NULL	NULL	NULL	In vivo hyperoxic exposure 	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In vivo hyperoxic exposure increases cultured lung fibroblast proliferation and c-Ha-ras expression .
	manualset3
94037	2	399521	13	NULL	NULL	0	NULL	increases	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo hyperoxic exposure increases cultured lung fibroblast proliferation and c-Ha-ras expression .
	manualset3
94039	3	399521	13	NULL	NULL	0	NULL	 lung fibroblast proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo hyperoxic exposure increases cultured lung fibroblast proliferation and c-Ha-ras expression .
	manualset3
94041	4	399521	13	NULL	NULL	0	NULL	c-Ha-ras expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo hyperoxic exposure increases cultured lung fibroblast proliferation and c-Ha-ras expression .
	manualset3
94146	1	399522	13	NULL	NULL	0	NULL	In vivo inoculation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo inoculation of a low metastatic BW 5147 derived T-cell lymphoma variant into syngeneic mice , had led to the generation of a highly metastatic variant .
	manualset3
94147	2	399522	13	NULL	NULL	0	NULL	low metastatic BW 5147 derived T-cell lymphoma variant	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo inoculation of a low metastatic BW 5147 derived T-cell lymphoma variant into syngeneic mice , had led to the generation of a highly metastatic variant .
	manualset3
94148	3	399522	13	NULL	NULL	0	NULL	syngeneic mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo inoculation of a low metastatic BW 5147 derived T-cell lymphoma variant into syngeneic mice , had led to the generation of a highly metastatic variant .
	manualset3
94149	4	399522	13	NULL	NULL	0	NULL	generation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo inoculation of a low metastatic BW 5147 derived T-cell lymphoma variant into syngeneic mice , had led to the generation of a highly metastatic variant .
	manualset3
94150	5	399522	13	NULL	NULL	0	NULL	metastatic variant 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo inoculation of a low metastatic BW 5147 derived T-cell lymphoma variant into syngeneic mice , had led to the generation of a highly metastatic variant .
	manualset3
94151	1	399523	13	NULL	NULL	0	NULL	In vivo modulation of G proteins	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo modulation of G proteins and opioid receptor function by antisense oligodeoxynucleotides .
	manualset3
94152	2	399523	13	NULL	NULL	0	NULL	opioid receptor function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo modulation of G proteins and opioid receptor function by antisense oligodeoxynucleotides .
	manualset3
94153	3	399523	13	NULL	NULL	0	NULL	antisense oligodeoxynucleotides	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo modulation of G proteins and opioid receptor function by antisense oligodeoxynucleotides .
	manualset3
94154	1	399524	13	NULL	NULL	0	NULL	In vivo occupancy	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo occupancy of the striatal dopamine uptake complex by various inhibitors does not predict their effects on locomotion .
	manualset3
94155	2	399524	13	NULL	NULL	NULL	NULL	 striatal dopamine uptake complex	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In vivo occupancy of the striatal dopamine uptake complex by various inhibitors does not predict their effects on locomotion .
	manualset3
94156	3	399524	13	NULL	NULL	0	NULL	various inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo occupancy of the striatal dopamine uptake complex by various inhibitors does not predict their effects on locomotion .
	manualset3
94157	4	399524	13	NULL	NULL	NULL	NULL	 effects	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In vivo occupancy of the striatal dopamine uptake complex by various inhibitors does not predict their effects on locomotion .
	manualset3
94158	5	399524	13	NULL	NULL	0	NULL	locomotion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo occupancy of the striatal dopamine uptake complex by various inhibitors does not predict their effects on locomotion .
	manualset3
94159	1	399525	13	NULL	NULL	0	NULL	In vivo solutions of thrombin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo solutions of thrombin were infused stereotactically into the right basal ganglia of rats .
	manualset3
94160	2	399525	13	NULL	NULL	NULL	NULL	right basal ganglia of rats	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In vivo solutions of thrombin were infused stereotactically into the right basal ganglia of rats .
	manualset3
94161	1	399526	13	NULL	NULL	0	NULL	In vivo study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo study showed that the expression of GM-CSF by RVJSB1175D/GM-CSF did not interfere with the HSV-1gD antibody production .
	manualset3
94162	2	399526	13	NULL	NULL	0	NULL	expression of GM-CSF 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo study showed that the expression of GM-CSF by RVJSB1175D/GM-CSF did not interfere with the HSV-1gD antibody production .
	manualset3
94163	3	399526	13	NULL	NULL	0	NULL	RVJSB1175D/GM-CSF 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo study showed that the expression of GM-CSF by RVJSB1175D/GM-CSF did not interfere with the HSV-1gD antibody production .
	manualset3
94164	4	399526	13	NULL	NULL	0	NULL	HSV-1gD antibody production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo study showed that the expression of GM-CSF by RVJSB1175D/GM-CSF did not interfere with the HSV-1gD antibody production .
	manualset3
94165	1	399527	13	NULL	NULL	0	NULL	In vivo therapeutic gas delivery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo therapeutic gas delivery for neuroprotection with echogenic liposomes .
	manualset3
94166	2	399527	13	NULL	NULL	0	NULL	neuroprotection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo therapeutic gas delivery for neuroprotection with echogenic liposomes .
	manualset3
94167	3	399527	13	NULL	NULL	0	NULL	echogenic liposomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo therapeutic gas delivery for neuroprotection with echogenic liposomes .
	manualset3
94168	1	399528	13	NULL	NULL	0	NULL	In situ electron holography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In situ electron holography showed that the oxide underwent reduction at elevated temperatures in a vacuum and was consequently reoxidized upon exposure to an oxygen flux at the same temperature .
	manualset3
94169	2	399528	13	NULL	NULL	0	NULL	oxide	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In situ electron holography showed that the oxide underwent reduction at elevated temperatures in a vacuum and was consequently reoxidized upon exposure to an oxygen flux at the same temperature .
	manualset3
94170	3	399528	13	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In situ electron holography showed that the oxide underwent reduction at elevated temperatures in a vacuum and was consequently reoxidized upon exposure to an oxygen flux at the same temperature .
	manualset3
94171	4	399528	13	NULL	NULL	0	NULL	temperatures 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In situ electron holography showed that the oxide underwent reduction at elevated temperatures in a vacuum and was consequently reoxidized upon exposure to an oxygen flux at the same temperature .
	manualset3
94172	5	399528	13	NULL	NULL	0	NULL	vacuum	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In situ electron holography showed that the oxide underwent reduction at elevated temperatures in a vacuum and was consequently reoxidized upon exposure to an oxygen flux at the same temperature .
	manualset3
94173	6	399528	13	NULL	NULL	0	NULL	exposure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In situ electron holography showed that the oxide underwent reduction at elevated temperatures in a vacuum and was consequently reoxidized upon exposure to an oxygen flux at the same temperature .
	manualset3
94174	7	399528	13	NULL	NULL	0	NULL	oxygen flux 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In situ electron holography showed that the oxide underwent reduction at elevated temperatures in a vacuum and was consequently reoxidized upon exposure to an oxygen flux at the same temperature .
	manualset3
94175	8	399528	13	NULL	NULL	0	NULL	temperature	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In situ electron holography showed that the oxide underwent reduction at elevated temperatures in a vacuum and was consequently reoxidized upon exposure to an oxygen flux at the same temperature .
	manualset3
94176	1	399529	13	NULL	NULL	0	NULL	Angiographic diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Angiographic diagnosis of combined injuries of the spleen and left kidney ) .
	manualset3
94177	2	399529	13	NULL	NULL	0	NULL	injuries of the spleen	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Angiographic diagnosis of combined injuries of the spleen and left kidney ) .
	manualset3
94178	3	399529	13	NULL	NULL	0	NULL	injuries of the left kidney	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Angiographic diagnosis of combined injuries of the spleen and left kidney ) .
	manualset3
94179	1	399530	13	NULL	NULL	0	NULL	Tokyo	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Tokyo ) 86 , 79-86 ) and to the submandibular proline-rich protein precursor MSG1 of the mouse ( D. Tronik-Le Roux , M. Senorale-Pose , and F. Rougeon , manuscript in preparation ) .
	manualset3
94180	2	399530	13	NULL	NULL	0	NULL	86 , 79-86 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( Tokyo ) 86 , 79-86 ) and to the submandibular proline-rich protein precursor MSG1 of the mouse ( D. Tronik-Le Roux , M. Senorale-Pose , and F. Rougeon , manuscript in preparation ) .
	manualset3
94181	3	399530	13	NULL	NULL	0	NULL	submandibular proline-rich protein precursor MSG1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Tokyo ) 86 , 79-86 ) and to the submandibular proline-rich protein precursor MSG1 of the mouse ( D. Tronik-Le Roux , M. Senorale-Pose , and F. Rougeon , manuscript in preparation ) .
	manualset3
94182	4	399530	13	NULL	NULL	0	NULL	mouse	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Tokyo ) 86 , 79-86 ) and to the submandibular proline-rich protein precursor MSG1 of the mouse ( D. Tronik-Le Roux , M. Senorale-Pose , and F. Rougeon , manuscript in preparation ) .
	manualset3
94183	5	399530	13	NULL	NULL	0	NULL	 D. Tronik-Le Roux	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( Tokyo ) 86 , 79-86 ) and to the submandibular proline-rich protein precursor MSG1 of the mouse ( D. Tronik-Le Roux , M. Senorale-Pose , and F. Rougeon , manuscript in preparation ) .
	manualset3
94184	6	399530	13	NULL	NULL	0	NULL	M. Senorale-Pose	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( Tokyo ) 86 , 79-86 ) and to the submandibular proline-rich protein precursor MSG1 of the mouse ( D. Tronik-Le Roux , M. Senorale-Pose , and F. Rougeon , manuscript in preparation ) .
	manualset3
94185	7	399530	13	NULL	NULL	0	NULL	F. Rougeon	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( Tokyo ) 86 , 79-86 ) and to the submandibular proline-rich protein precursor MSG1 of the mouse ( D. Tronik-Le Roux , M. Senorale-Pose , and F. Rougeon , manuscript in preparation ) .
	manualset3
94186	8	399530	13	NULL	NULL	0	NULL	manuscript	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Tokyo ) 86 , 79-86 ) and to the submandibular proline-rich protein precursor MSG1 of the mouse ( D. Tronik-Le Roux , M. Senorale-Pose , and F. Rougeon , manuscript in preparation ) .
	manualset3
94187	9	399530	13	NULL	NULL	0	NULL	preparation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Tokyo ) 86 , 79-86 ) and to the submandibular proline-rich protein precursor MSG1 of the mouse ( D. Tronik-Le Roux , M. Senorale-Pose , and F. Rougeon , manuscript in preparation ) .
	manualset3
86664	1	399531	5	NULL	NULL	0	NULL	In situ hybridization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In situ hybridization shows that MeHsp90 is highly expressed in previtellogenic oocytes and its expression decreases with the progress of maturation , and finally stops in late-vitellogenic oocytes .
	manualset3
86665	2	399531	5	NULL	NULL	0	NULL	MeHsp90	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In situ hybridization shows that MeHsp90 is highly expressed in previtellogenic oocytes and its expression decreases with the progress of maturation , and finally stops in late-vitellogenic oocytes .
	manualset3
86666	3	399531	5	NULL	NULL	0	NULL	previtellogenic oocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In situ hybridization shows that MeHsp90 is highly expressed in previtellogenic oocytes and its expression decreases with the progress of maturation , and finally stops in late-vitellogenic oocytes .
	manualset3
86667	4	399531	5	NULL	NULL	NULL	NULL	expression	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In situ hybridization shows that MeHsp90 is highly expressed in previtellogenic oocytes and its expression decreases with the progress of maturation , and finally stops in late-vitellogenic oocytes .
	manualset3
86668	5	399531	5	NULL	NULL	0	NULL	progress	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In situ hybridization shows that MeHsp90 is highly expressed in previtellogenic oocytes and its expression decreases with the progress of maturation , and finally stops in late-vitellogenic oocytes .
	manualset3
86669	6	399531	5	NULL	NULL	0	NULL	maturation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In situ hybridization shows that MeHsp90 is highly expressed in previtellogenic oocytes and its expression decreases with the progress of maturation , and finally stops in late-vitellogenic oocytes .
	manualset3
86670	7	399531	5	NULL	NULL	0	NULL	late-vitellogenic oocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In situ hybridization shows that MeHsp90 is highly expressed in previtellogenic oocytes and its expression decreases with the progress of maturation , and finally stops in late-vitellogenic oocytes .
	manualset3
86671	1	399532	5	NULL	NULL	0	NULL	In situ proteomic profiling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In situ proteomic profiling of tumors is a powerful technology with potential to enhance our understanding of tumor biology , but sources of variability due to patient and tumor heterogeneity are poorly understood and are the topic of this investigation .
	manualset3
86672	2	399532	5	NULL	NULL	0	NULL	tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In situ proteomic profiling of tumors is a powerful technology with potential to enhance our understanding of tumor biology , but sources of variability due to patient and tumor heterogeneity are poorly understood and are the topic of this investigation .
	manualset3
86673	3	399532	5	NULL	NULL	0	NULL	powerful technology	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In situ proteomic profiling of tumors is a powerful technology with potential to enhance our understanding of tumor biology , but sources of variability due to patient and tumor heterogeneity are poorly understood and are the topic of this investigation .
	manualset3
86674	4	399532	5	NULL	NULL	0	NULL	tumor biology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In situ proteomic profiling of tumors is a powerful technology with potential to enhance our understanding of tumor biology , but sources of variability due to patient and tumor heterogeneity are poorly understood and are the topic of this investigation .
	manualset3
86675	5	399532	5	NULL	NULL	0	NULL	variability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In situ proteomic profiling of tumors is a powerful technology with potential to enhance our understanding of tumor biology , but sources of variability due to patient and tumor heterogeneity are poorly understood and are the topic of this investigation .
	manualset3
86676	6	399532	5	NULL	NULL	0	NULL	patient	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In situ proteomic profiling of tumors is a powerful technology with potential to enhance our understanding of tumor biology , but sources of variability due to patient and tumor heterogeneity are poorly understood and are the topic of this investigation .
	manualset3
86677	7	399532	5	NULL	NULL	0	NULL	tumor heterogeneity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In situ proteomic profiling of tumors is a powerful technology with potential to enhance our understanding of tumor biology , but sources of variability due to patient and tumor heterogeneity are poorly understood and are the topic of this investigation .
	manualset3
86678	8	399532	5	NULL	NULL	0	NULL	investigation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In situ proteomic profiling of tumors is a powerful technology with potential to enhance our understanding of tumor biology , but sources of variability due to patient and tumor heterogeneity are poorly understood and are the topic of this investigation .
	manualset3
86679	1	399533	5	NULL	NULL	NULL	NULL	In situ steady-state , single-pass small intestine perfusions	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In situ steady-state , single-pass small intestine perfusions in rats were carried out to compare the effect of the bicarbonate and citrate World Health Organization oral rehydration solutions and a base precursor-free solution on intestinal water and electrolyte transport after inducing intestinal secretion with purified heat-stable Escherichia coli enterotoxin .
	manualset3
86680	2	399533	5	NULL	NULL	NULL	NULL	rats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In situ steady-state , single-pass small intestine perfusions in rats were carried out to compare the effect of the bicarbonate and citrate World Health Organization oral rehydration solutions and a base precursor-free solution on intestinal water and electrolyte transport after inducing intestinal secretion with purified heat-stable Escherichia coli enterotoxin .
	manualset3
86681	3	399533	5	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In situ steady-state , single-pass small intestine perfusions in rats were carried out to compare the effect of the bicarbonate and citrate World Health Organization oral rehydration solutions and a base precursor-free solution on intestinal water and electrolyte transport after inducing intestinal secretion with purified heat-stable Escherichia coli enterotoxin .
	manualset3
86682	4	399533	5	NULL	NULL	NULL	NULL	bicarbonate and citrate World Health Organization oral rehydration solutions	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In situ steady-state , single-pass small intestine perfusions in rats were carried out to compare the effect of the bicarbonate and citrate World Health Organization oral rehydration solutions and a base precursor-free solution on intestinal water and electrolyte transport after inducing intestinal secretion with purified heat-stable Escherichia coli enterotoxin .
	manualset3
86683	5	399533	5	NULL	NULL	NULL	NULL	base precursor-free solution	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In situ steady-state , single-pass small intestine perfusions in rats were carried out to compare the effect of the bicarbonate and citrate World Health Organization oral rehydration solutions and a base precursor-free solution on intestinal water and electrolyte transport after inducing intestinal secretion with purified heat-stable Escherichia coli enterotoxin .
	manualset3
86684	6	399533	5	NULL	NULL	0	NULL	intestinal water and electrolyte transport	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In situ steady-state , single-pass small intestine perfusions in rats were carried out to compare the effect of the bicarbonate and citrate World Health Organization oral rehydration solutions and a base precursor-free solution on intestinal water and electrolyte transport after inducing intestinal secretion with purified heat-stable Escherichia coli enterotoxin .
	manualset3
86685	7	399533	5	NULL	NULL	NULL	NULL	intestinal secretion	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In situ steady-state , single-pass small intestine perfusions in rats were carried out to compare the effect of the bicarbonate and citrate World Health Organization oral rehydration solutions and a base precursor-free solution on intestinal water and electrolyte transport after inducing intestinal secretion with purified heat-stable Escherichia coli enterotoxin .
	manualset3
86686	8	399533	5	NULL	NULL	0	NULL	purified heat-stable Escherichia coli enterotoxin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In situ steady-state , single-pass small intestine perfusions in rats were carried out to compare the effect of the bicarbonate and citrate World Health Organization oral rehydration solutions and a base precursor-free solution on intestinal water and electrolyte transport after inducing intestinal secretion with purified heat-stable Escherichia coli enterotoxin .
	manualset3
86687	1	399534	5	NULL	NULL	NULL	NULL	1904	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In 1904 , James Collier became the first to describe cerebellar tonsillar herniation as a `` false localizing sign '' often associated with intracranial tumors .
	manualset3
86688	2	399534	5	NULL	NULL	0	NULL	James Collier	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1904 , James Collier became the first to describe cerebellar tonsillar herniation as a `` false localizing sign '' often associated with intracranial tumors .
	manualset3
86689	3	399534	5	NULL	NULL	0	NULL	cerebellar tonsillar herniation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1904 , James Collier became the first to describe cerebellar tonsillar herniation as a `` false localizing sign '' often associated with intracranial tumors .
	manualset3
86690	4	399534	5	NULL	NULL	0	NULL	false localizing sign	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1904 , James Collier became the first to describe cerebellar tonsillar herniation as a `` false localizing sign '' often associated with intracranial tumors .
	manualset3
86691	5	399534	5	NULL	NULL	0	NULL	intracranial tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1904 , James Collier became the first to describe cerebellar tonsillar herniation as a `` false localizing sign '' often associated with intracranial tumors .
	manualset3
86692	1	399535	5	NULL	NULL	NULL	NULL	1969	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In 1969 , five cases of melioidosis in three separate outbreaks were diagnosed in nonhuman primates in the United States .
	manualset3
86693	2	399535	5	NULL	NULL	0	NULL	five cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1969 , five cases of melioidosis in three separate outbreaks were diagnosed in nonhuman primates in the United States .
	manualset3
86694	3	399535	5	NULL	NULL	0	NULL	melioidosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1969 , five cases of melioidosis in three separate outbreaks were diagnosed in nonhuman primates in the United States .
	manualset3
86695	4	399535	5	NULL	NULL	0	NULL	three separate outbreaks	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1969 , five cases of melioidosis in three separate outbreaks were diagnosed in nonhuman primates in the United States .
	manualset3
86696	5	399535	5	NULL	NULL	0	NULL	nonhuman primates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1969 , five cases of melioidosis in three separate outbreaks were diagnosed in nonhuman primates in the United States .
	manualset3
86697	6	399535	5	NULL	NULL	0	NULL	United States	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1969 , five cases of melioidosis in three separate outbreaks were diagnosed in nonhuman primates in the United States .
	manualset3
86698	1	399536	5	NULL	NULL	0	NULL	1977	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1977 , Fisher reported that in patients with possible normal-pressure hydrocephalus ( NPH ) , if the gait abnormality preceded dementia , surgery usually had a favorable outcome and vice versa .
	manualset3
86699	2	399536	5	NULL	NULL	0	NULL	Fisher	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1977 , Fisher reported that in patients with possible normal-pressure hydrocephalus ( NPH ) , if the gait abnormality preceded dementia , surgery usually had a favorable outcome and vice versa .
	manualset3
86700	3	399536	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1977 , Fisher reported that in patients with possible normal-pressure hydrocephalus ( NPH ) , if the gait abnormality preceded dementia , surgery usually had a favorable outcome and vice versa .
	manualset3
86701	4	399536	5	NULL	NULL	0	NULL	normal-pressure hydrocephalus ( NPH )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1977 , Fisher reported that in patients with possible normal-pressure hydrocephalus ( NPH ) , if the gait abnormality preceded dementia , surgery usually had a favorable outcome and vice versa .
	manualset3
86702	5	399536	5	NULL	NULL	0	NULL	gait abnormality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1977 , Fisher reported that in patients with possible normal-pressure hydrocephalus ( NPH ) , if the gait abnormality preceded dementia , surgery usually had a favorable outcome and vice versa .
	manualset3
86703	6	399536	5	NULL	NULL	0	NULL	dementia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1977 , Fisher reported that in patients with possible normal-pressure hydrocephalus ( NPH ) , if the gait abnormality preceded dementia , surgery usually had a favorable outcome and vice versa .
	manualset3
86704	7	399536	5	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1977 , Fisher reported that in patients with possible normal-pressure hydrocephalus ( NPH ) , if the gait abnormality preceded dementia , surgery usually had a favorable outcome and vice versa .
	manualset3
86705	8	399536	5	NULL	NULL	0	NULL	favorable outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1977 , Fisher reported that in patients with possible normal-pressure hydrocephalus ( NPH ) , if the gait abnormality preceded dementia , surgery usually had a favorable outcome and vice versa .
	manualset3
86706	1	399537	5	NULL	NULL	0	NULL	2004	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	In 2004 , Florida accounted for 11 % of the total number of acquired immunodeficiency syndrome ( AIDS ) cases in the United States , ranking third behind New York and California .
	manualset3
86707	2	399537	5	NULL	NULL	NULL	NULL	Florida	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In 2004 , Florida accounted for 11 % of the total number of acquired immunodeficiency syndrome ( AIDS ) cases in the United States , ranking third behind New York and California .
	manualset3
86708	3	399537	5	NULL	NULL	0	NULL	11 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In 2004 , Florida accounted for 11 % of the total number of acquired immunodeficiency syndrome ( AIDS ) cases in the United States , ranking third behind New York and California .
	manualset3
86709	4	399537	5	NULL	NULL	0	NULL	acquired immunodeficiency syndrome ( AIDS ) cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 2004 , Florida accounted for 11 % of the total number of acquired immunodeficiency syndrome ( AIDS ) cases in the United States , ranking third behind New York and California .
	manualset3
86710	5	399537	5	NULL	NULL	0	NULL	United States	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In 2004 , Florida accounted for 11 % of the total number of acquired immunodeficiency syndrome ( AIDS ) cases in the United States , ranking third behind New York and California .
	manualset3
86711	6	399537	5	NULL	NULL	0	NULL	New York	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In 2004 , Florida accounted for 11 % of the total number of acquired immunodeficiency syndrome ( AIDS ) cases in the United States , ranking third behind New York and California .
	manualset3
86712	7	399537	5	NULL	NULL	0	NULL	California	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In 2004 , Florida accounted for 11 % of the total number of acquired immunodeficiency syndrome ( AIDS ) cases in the United States , ranking third behind New York and California .
	manualset3
86713	1	399538	5	NULL	NULL	0	NULL	2008	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	In 2008 , patients in the intensive care unit ( ICU ) at Danbury Hospital , Danbury , Connecticut , experienced 79 pressure ulcers .
	manualset3
86714	2	399538	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 2008 , patients in the intensive care unit ( ICU ) at Danbury Hospital , Danbury , Connecticut , experienced 79 pressure ulcers .
	manualset3
86715	3	399538	5	NULL	NULL	0	NULL	intensive care unit ( ICU )	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In 2008 , patients in the intensive care unit ( ICU ) at Danbury Hospital , Danbury , Connecticut , experienced 79 pressure ulcers .
	manualset3
86716	4	399538	5	NULL	NULL	0	NULL	Danbury Hospital	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In 2008 , patients in the intensive care unit ( ICU ) at Danbury Hospital , Danbury , Connecticut , experienced 79 pressure ulcers .
	manualset3
86717	5	399538	5	NULL	NULL	0	NULL	Danbury	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In 2008 , patients in the intensive care unit ( ICU ) at Danbury Hospital , Danbury , Connecticut , experienced 79 pressure ulcers .
	manualset3
86718	6	399538	5	NULL	NULL	0	NULL	Connecticut	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In 2008 , patients in the intensive care unit ( ICU ) at Danbury Hospital , Danbury , Connecticut , experienced 79 pressure ulcers .
	manualset3
86719	7	399538	5	NULL	NULL	0	NULL	79 pressure ulcers	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 2008 , patients in the intensive care unit ( ICU ) at Danbury Hospital , Danbury , Connecticut , experienced 79 pressure ulcers .
	manualset3
86720	1	399539	5	NULL	NULL	0	NULL	7 ( 50 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In 7 ( 50 % ) biological signs of pancreatitis were noted : mean amylase level 81 IU ( range 30-201 IU , normal value less than 40 IU ) , mean lipase level 949 IU ( range 468-2 , 000 IU , normal value less than 300 IU ) .
	manualset3
86721	2	399539	5	NULL	NULL	0	NULL	biological signs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 7 ( 50 % ) biological signs of pancreatitis were noted : mean amylase level 81 IU ( range 30-201 IU , normal value less than 40 IU ) , mean lipase level 949 IU ( range 468-2 , 000 IU , normal value less than 300 IU ) .
	manualset3
86722	3	399539	5	NULL	NULL	0	NULL	pancreatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In 7 ( 50 % ) biological signs of pancreatitis were noted : mean amylase level 81 IU ( range 30-201 IU , normal value less than 40 IU ) , mean lipase level 949 IU ( range 468-2 , 000 IU , normal value less than 300 IU ) .
	manualset3
86723	4	399539	5	NULL	NULL	0	NULL	mean amylase level 81 IU ( range 30-201 IU , normal value less than 40 IU )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 7 ( 50 % ) biological signs of pancreatitis were noted : mean amylase level 81 IU ( range 30-201 IU , normal value less than 40 IU ) , mean lipase level 949 IU ( range 468-2 , 000 IU , normal value less than 300 IU ) .
	manualset3
86724	5	399539	5	NULL	NULL	0	NULL	mean lipase level 949 IU ( range 468-2 , 000 IU , normal value less than 300 IU )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 7 ( 50 % ) biological signs of pancreatitis were noted : mean amylase level 81 IU ( range 30-201 IU , normal value less than 40 IU ) , mean lipase level 949 IU ( range 468-2 , 000 IU , normal value less than 300 IU ) .
	manualset3
86725	1	399540	5	NULL	NULL	0	NULL	expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In ALL , the expression of CD58 was inversely correlated with the presence of a clinical tumoral syndrome ( p = 0.0009 ) , leucocytosis ( p = 0.005 ) , and the percent of peripheral blast cells ( p = 0.001 ) .
	manualset3
86726	2	399540	5	NULL	NULL	0	NULL	CD58	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In ALL , the expression of CD58 was inversely correlated with the presence of a clinical tumoral syndrome ( p = 0.0009 ) , leucocytosis ( p = 0.005 ) , and the percent of peripheral blast cells ( p = 0.001 ) .
	manualset3
86727	3	399540	5	NULL	NULL	0	NULL	clinical tumoral syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In ALL , the expression of CD58 was inversely correlated with the presence of a clinical tumoral syndrome ( p = 0.0009 ) , leucocytosis ( p = 0.005 ) , and the percent of peripheral blast cells ( p = 0.001 ) .
	manualset3
86728	4	399540	5	NULL	NULL	0	NULL	( p = 0.0009 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In ALL , the expression of CD58 was inversely correlated with the presence of a clinical tumoral syndrome ( p = 0.0009 ) , leucocytosis ( p = 0.005 ) , and the percent of peripheral blast cells ( p = 0.001 ) .
	manualset3
86729	5	399540	5	NULL	NULL	0	NULL	leucocytosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In ALL , the expression of CD58 was inversely correlated with the presence of a clinical tumoral syndrome ( p = 0.0009 ) , leucocytosis ( p = 0.005 ) , and the percent of peripheral blast cells ( p = 0.001 ) .
	manualset3
86730	6	399540	5	NULL	NULL	0	NULL	( p = 0.005 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In ALL , the expression of CD58 was inversely correlated with the presence of a clinical tumoral syndrome ( p = 0.0009 ) , leucocytosis ( p = 0.005 ) , and the percent of peripheral blast cells ( p = 0.001 ) .
	manualset3
86732	7	399540	5	NULL	NULL	0	NULL	peripheral blast cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In ALL , the expression of CD58 was inversely correlated with the presence of a clinical tumoral syndrome ( p = 0.0009 ) , leucocytosis ( p = 0.005 ) , and the percent of peripheral blast cells ( p = 0.001 ) .
	manualset3
86733	8	399540	5	NULL	NULL	0	NULL	( p = 0.001 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In ALL , the expression of CD58 was inversely correlated with the presence of a clinical tumoral syndrome ( p = 0.0009 ) , leucocytosis ( p = 0.005 ) , and the percent of peripheral blast cells ( p = 0.001 ) .
	manualset3
86734	1	399541	5	NULL	NULL	0	NULL	Brazil	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In Brazil , nursing professionals are trained based on the perspective of professional competencies .
	manualset3
86735	2	399541	5	NULL	NULL	0	NULL	nursing professionals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In Brazil , nursing professionals are trained based on the perspective of professional competencies .
	manualset3
86736	3	399541	5	NULL	NULL	0	NULL	perspective	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In Brazil , nursing professionals are trained based on the perspective of professional competencies .
	manualset3
86737	4	399541	5	NULL	NULL	0	NULL	professional competencies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In Brazil , nursing professionals are trained based on the perspective of professional competencies .
	manualset3
86739	1	399542	5	NULL	NULL	0	NULL	Canada	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In Canada , provincial and territorial laws address circumstances in which a substitute decision-maker may be appointed for an adult deemed legally incapable of making decisions in one or more areas of life .
	manualset3
86742	2	399542	5	NULL	NULL	0	NULL	provincial and territorial laws	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In Canada , provincial and territorial laws address circumstances in which a substitute decision-maker may be appointed for an adult deemed legally incapable of making decisions in one or more areas of life .
	manualset3
86745	3	399542	5	NULL	NULL	0	NULL	circumstances	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In Canada , provincial and territorial laws address circumstances in which a substitute decision-maker may be appointed for an adult deemed legally incapable of making decisions in one or more areas of life .
	manualset3
86747	4	399542	5	NULL	NULL	0	NULL	substitute decision-maker	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In Canada , provincial and territorial laws address circumstances in which a substitute decision-maker may be appointed for an adult deemed legally incapable of making decisions in one or more areas of life .
	manualset3
86748	5	399542	5	NULL	NULL	0	NULL	adult	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In Canada , provincial and territorial laws address circumstances in which a substitute decision-maker may be appointed for an adult deemed legally incapable of making decisions in one or more areas of life .
	manualset3
86751	6	399542	5	NULL	NULL	0	NULL	making decisions	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In Canada , provincial and territorial laws address circumstances in which a substitute decision-maker may be appointed for an adult deemed legally incapable of making decisions in one or more areas of life .
	manualset3
86753	7	399542	5	NULL	NULL	NULL	NULL	life	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In Canada , provincial and territorial laws address circumstances in which a substitute decision-maker may be appointed for an adult deemed legally incapable of making decisions in one or more areas of life .
	manualset3
86754	1	399543	5	NULL	NULL	0	NULL	France	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In France , it is the official Veterinary Services who are responsible for food safety and who must respond to these demands .
	manualset3
86756	2	399543	5	NULL	NULL	0	NULL	 official Veterinary Services	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In France , it is the official Veterinary Services who are responsible for food safety and who must respond to these demands .
	manualset3
86757	3	399543	5	NULL	NULL	0	NULL	food safety	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In France , it is the official Veterinary Services who are responsible for food safety and who must respond to these demands .
	manualset3
86760	1	399544	5	NULL	NULL	0	NULL	France	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In France and in other European countries , however , a particular effect was observed early on that received various labels : disinhibitor , stimulant , antiautistic and anti-deficit , and that involved the beneficial action of certain neuroleptics on the negative symptoms of schizophrenia .
	manualset3
86761	2	399544	5	NULL	NULL	0	NULL	European countries	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In France and in other European countries , however , a particular effect was observed early on that received various labels : disinhibitor , stimulant , antiautistic and anti-deficit , and that involved the beneficial action of certain neuroleptics on the negative symptoms of schizophrenia .
	manualset3
86762	3	399544	5	NULL	NULL	0	NULL	particular effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In France and in other European countries , however , a particular effect was observed early on that received various labels : disinhibitor , stimulant , antiautistic and anti-deficit , and that involved the beneficial action of certain neuroleptics on the negative symptoms of schizophrenia .
	manualset3
86763	4	399544	5	NULL	NULL	0	NULL	disinhibitor	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In France and in other European countries , however , a particular effect was observed early on that received various labels : disinhibitor , stimulant , antiautistic and anti-deficit , and that involved the beneficial action of certain neuroleptics on the negative symptoms of schizophrenia .
	manualset3
86764	5	399544	5	NULL	NULL	0	NULL	stimulant	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In France and in other European countries , however , a particular effect was observed early on that received various labels : disinhibitor , stimulant , antiautistic and anti-deficit , and that involved the beneficial action of certain neuroleptics on the negative symptoms of schizophrenia .
	manualset3
86767	6	399544	5	NULL	NULL	NULL	NULL	antiautistic	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In France and in other European countries , however , a particular effect was observed early on that received various labels : disinhibitor , stimulant , antiautistic and anti-deficit , and that involved the beneficial action of certain neuroleptics on the negative symptoms of schizophrenia .
	manualset3
86768	7	399544	5	NULL	NULL	0	NULL	beneficial action	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In France and in other European countries , however , a particular effect was observed early on that received various labels : disinhibitor , stimulant , antiautistic and anti-deficit , and that involved the beneficial action of certain neuroleptics on the negative symptoms of schizophrenia .
	manualset3
86769	8	399544	5	NULL	NULL	0	NULL	neuroleptics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In France and in other European countries , however , a particular effect was observed early on that received various labels : disinhibitor , stimulant , antiautistic and anti-deficit , and that involved the beneficial action of certain neuroleptics on the negative symptoms of schizophrenia .
	manualset3
86770	9	399544	5	NULL	NULL	0	NULL	negative symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In France and in other European countries , however , a particular effect was observed early on that received various labels : disinhibitor , stimulant , antiautistic and anti-deficit , and that involved the beneficial action of certain neuroleptics on the negative symptoms of schizophrenia .
	manualset3
86773	10	399544	5	NULL	NULL	0	NULL	schizophrenia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In France and in other European countries , however , a particular effect was observed early on that received various labels : disinhibitor , stimulant , antiautistic and anti-deficit , and that involved the beneficial action of certain neuroleptics on the negative symptoms of schizophrenia .
	manualset3
89564	11	399544	5	NULL	NULL	0	NULL	anti-deficit	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In France and in other European countries , however , a particular effect was observed early on that received various labels : disinhibitor , stimulant , antiautistic and anti-deficit , and that involved the beneficial action of certain neuroleptics on the negative symptoms of schizophrenia .
	manualset3
86774	1	399545	5	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Too many women currently live in danger ) .
	manualset3
86779	1	399546	5	NULL	NULL	0	NULL	Kanto	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In Kanto , Kinki and Chugoku/Shikoku Districts , however , proportion of atherothrombotic stroke was larger than that of lacunar stroke , which seemed to correspond to the higher frequency of patients with diabetes mellitus and hyperlipidemia in these 3 districts .
	manualset3
86780	2	399546	5	NULL	NULL	0	NULL	Kinki	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In Kanto , Kinki and Chugoku/Shikoku Districts , however , proportion of atherothrombotic stroke was larger than that of lacunar stroke , which seemed to correspond to the higher frequency of patients with diabetes mellitus and hyperlipidemia in these 3 districts .
	manualset3
86783	3	399546	5	NULL	NULL	0	NULL	Chugoku/Shikoku Districts	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In Kanto , Kinki and Chugoku/Shikoku Districts , however , proportion of atherothrombotic stroke was larger than that of lacunar stroke , which seemed to correspond to the higher frequency of patients with diabetes mellitus and hyperlipidemia in these 3 districts .
	manualset3
86784	4	399546	5	NULL	NULL	0	NULL	atherothrombotic stroke	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In Kanto , Kinki and Chugoku/Shikoku Districts , however , proportion of atherothrombotic stroke was larger than that of lacunar stroke , which seemed to correspond to the higher frequency of patients with diabetes mellitus and hyperlipidemia in these 3 districts .
	manualset3
86787	5	399546	5	NULL	NULL	0	NULL	lacunar stroke	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In Kanto , Kinki and Chugoku/Shikoku Districts , however , proportion of atherothrombotic stroke was larger than that of lacunar stroke , which seemed to correspond to the higher frequency of patients with diabetes mellitus and hyperlipidemia in these 3 districts .
	manualset3
86795	6	399546	5	NULL	NULL	0	NULL	higher frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In Kanto , Kinki and Chugoku/Shikoku Districts , however , proportion of atherothrombotic stroke was larger than that of lacunar stroke , which seemed to correspond to the higher frequency of patients with diabetes mellitus and hyperlipidemia in these 3 districts .
	manualset3
86798	7	399546	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In Kanto , Kinki and Chugoku/Shikoku Districts , however , proportion of atherothrombotic stroke was larger than that of lacunar stroke , which seemed to correspond to the higher frequency of patients with diabetes mellitus and hyperlipidemia in these 3 districts .
	manualset3
86801	8	399546	5	NULL	NULL	0	NULL	diabetes mellitus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In Kanto , Kinki and Chugoku/Shikoku Districts , however , proportion of atherothrombotic stroke was larger than that of lacunar stroke , which seemed to correspond to the higher frequency of patients with diabetes mellitus and hyperlipidemia in these 3 districts .
	manualset3
86805	9	399546	5	NULL	NULL	0	NULL	hyperlipidemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In Kanto , Kinki and Chugoku/Shikoku Districts , however , proportion of atherothrombotic stroke was larger than that of lacunar stroke , which seemed to correspond to the higher frequency of patients with diabetes mellitus and hyperlipidemia in these 3 districts .
	manualset3
86807	10	399546	5	NULL	NULL	0	NULL	3 districts	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In Kanto , Kinki and Chugoku/Shikoku Districts , however , proportion of atherothrombotic stroke was larger than that of lacunar stroke , which seemed to correspond to the higher frequency of patients with diabetes mellitus and hyperlipidemia in these 3 districts .
	manualset3
86808	1	399547	5	NULL	NULL	0	NULL	MM	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In MM , the percentage of BM infiltration and Ki-67 index were positively associated with TRF2 , TANK1 and hTERT expression ( P 0.03 ) and negatively with TL ( P = 0.02 ) , whereas lactate dehydrogenase was significantly correlated with TRF2 mRNA ( P = 0.008 ) .
	manualset3
86817	2	399547	5	NULL	NULL	0	NULL	BM infiltration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In MM , the percentage of BM infiltration and Ki-67 index were positively associated with TRF2 , TANK1 and hTERT expression ( P 0.03 ) and negatively with TL ( P = 0.02 ) , whereas lactate dehydrogenase was significantly correlated with TRF2 mRNA ( P = 0.008 ) .
	manualset3
86937	3	399547	5	NULL	NULL	0	NULL	Ki-67 index	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In MM , the percentage of BM infiltration and Ki-67 index were positively associated with TRF2 , TANK1 and hTERT expression ( P 0.03 ) and negatively with TL ( P = 0.02 ) , whereas lactate dehydrogenase was significantly correlated with TRF2 mRNA ( P = 0.008 ) .
	manualset3
86938	4	399547	5	NULL	NULL	0	NULL	TRF2 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In MM , the percentage of BM infiltration and Ki-67 index were positively associated with TRF2 , TANK1 and hTERT expression ( P 0.03 ) and negatively with TL ( P = 0.02 ) , whereas lactate dehydrogenase was significantly correlated with TRF2 mRNA ( P = 0.008 ) .
	manualset3
86939	5	399547	5	NULL	NULL	0	NULL	TANK1 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In MM , the percentage of BM infiltration and Ki-67 index were positively associated with TRF2 , TANK1 and hTERT expression ( P 0.03 ) and negatively with TL ( P = 0.02 ) , whereas lactate dehydrogenase was significantly correlated with TRF2 mRNA ( P = 0.008 ) .
	manualset3
86940	6	399547	5	NULL	NULL	0	NULL	hTERT expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In MM , the percentage of BM infiltration and Ki-67 index were positively associated with TRF2 , TANK1 and hTERT expression ( P 0.03 ) and negatively with TL ( P = 0.02 ) , whereas lactate dehydrogenase was significantly correlated with TRF2 mRNA ( P = 0.008 ) .
	manualset3
86941	7	399547	5	NULL	NULL	0	NULL	P 0.03	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In MM , the percentage of BM infiltration and Ki-67 index were positively associated with TRF2 , TANK1 and hTERT expression ( P 0.03 ) and negatively with TL ( P = 0.02 ) , whereas lactate dehydrogenase was significantly correlated with TRF2 mRNA ( P = 0.008 ) .
	manualset3
86942	8	399547	5	NULL	NULL	0	NULL	TL	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In MM , the percentage of BM infiltration and Ki-67 index were positively associated with TRF2 , TANK1 and hTERT expression ( P 0.03 ) and negatively with TL ( P = 0.02 ) , whereas lactate dehydrogenase was significantly correlated with TRF2 mRNA ( P = 0.008 ) .
	manualset3
86943	9	399547	5	NULL	NULL	NULL	NULL	P = 0.02	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In MM , the percentage of BM infiltration and Ki-67 index were positively associated with TRF2 , TANK1 and hTERT expression ( P 0.03 ) and negatively with TL ( P = 0.02 ) , whereas lactate dehydrogenase was significantly correlated with TRF2 mRNA ( P = 0.008 ) .
	manualset3
86944	10	399547	5	NULL	NULL	0	NULL	lactate dehydrogenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In MM , the percentage of BM infiltration and Ki-67 index were positively associated with TRF2 , TANK1 and hTERT expression ( P 0.03 ) and negatively with TL ( P = 0.02 ) , whereas lactate dehydrogenase was significantly correlated with TRF2 mRNA ( P = 0.008 ) .
	manualset3
86945	11	399547	5	NULL	NULL	0	NULL	TRF2 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In MM , the percentage of BM infiltration and Ki-67 index were positively associated with TRF2 , TANK1 and hTERT expression ( P 0.03 ) and negatively with TL ( P = 0.02 ) , whereas lactate dehydrogenase was significantly correlated with TRF2 mRNA ( P = 0.008 ) .
	manualset3
86946	12	399547	5	NULL	NULL	0	NULL	P = 0.008	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In MM , the percentage of BM infiltration and Ki-67 index were positively associated with TRF2 , TANK1 and hTERT expression ( P 0.03 ) and negatively with TL ( P = 0.02 ) , whereas lactate dehydrogenase was significantly correlated with TRF2 mRNA ( P = 0.008 ) .
	manualset3
86947	1	399548	5	NULL	NULL	NULL	NULL	P3	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In P3 , two out of nine amino acid changes occur in hydrophilic regions .
	manualset3
86948	2	399548	5	NULL	NULL	NULL	NULL	two out of nine amino acid changes	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In P3 , two out of nine amino acid changes occur in hydrophilic regions .
	manualset3
86949	3	399548	5	NULL	NULL	0	NULL	hydrophilic regions	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In P3 , two out of nine amino acid changes occur in hydrophilic regions .
	manualset3
86950	1	399549	5	NULL	NULL	NULL	NULL	PD	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In PD , ERC atrophy , as measured on MRI , however , has received less attention , compared to hippocampal atrophy .
	manualset3
86951	2	399549	5	NULL	NULL	0	NULL	ERC atrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In PD , ERC atrophy , as measured on MRI , however , has received less attention , compared to hippocampal atrophy .
	manualset3
86952	3	399549	5	NULL	NULL	NULL	NULL	MRI	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In PD , ERC atrophy , as measured on MRI , however , has received less attention , compared to hippocampal atrophy .
	manualset3
86953	4	399549	5	NULL	NULL	0	NULL	attention	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In PD , ERC atrophy , as measured on MRI , however , has received less attention , compared to hippocampal atrophy .
	manualset3
86954	5	399549	5	NULL	NULL	0	NULL	hippocampal atrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In PD , ERC atrophy , as measured on MRI , however , has received less attention , compared to hippocampal atrophy .
	manualset3
86955	1	399550	5	NULL	NULL	0	NULL	Spain	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In Spain , a close relationship has been found between the yearly rate of aminopenicillin consumption and penicillin resistance .
	manualset3
86956	2	399550	5	NULL	NULL	0	NULL	close relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In Spain , a close relationship has been found between the yearly rate of aminopenicillin consumption and penicillin resistance .
	manualset3
86957	3	399550	5	NULL	NULL	0	NULL	yearly rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In Spain , a close relationship has been found between the yearly rate of aminopenicillin consumption and penicillin resistance .
	manualset3
86958	4	399550	5	NULL	NULL	0	NULL	aminopenicillin consumption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In Spain , a close relationship has been found between the yearly rate of aminopenicillin consumption and penicillin resistance .
	manualset3
86959	5	399550	5	NULL	NULL	0	NULL	penicillin resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In Spain , a close relationship has been found between the yearly rate of aminopenicillin consumption and penicillin resistance .
	manualset3
86960	1	399551	5	NULL	NULL	0	NULL	Xenopus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In Xenopus , Cdk1 phosphorylates Emi2 and both destabilizes and inactivates it , whereas Mos recruits PP2A phosphatase to antagonize the Cdk1 phosphorylation .
	manualset3
86961	2	399551	5	NULL	NULL	0	NULL	Cdk1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In Xenopus , Cdk1 phosphorylates Emi2 and both destabilizes and inactivates it , whereas Mos recruits PP2A phosphatase to antagonize the Cdk1 phosphorylation .
	manualset3
86962	3	399551	5	NULL	NULL	0	NULL	Emi2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In Xenopus , Cdk1 phosphorylates Emi2 and both destabilizes and inactivates it , whereas Mos recruits PP2A phosphatase to antagonize the Cdk1 phosphorylation .
	manualset3
86963	4	399551	5	NULL	NULL	0	NULL	Mos	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In Xenopus , Cdk1 phosphorylates Emi2 and both destabilizes and inactivates it , whereas Mos recruits PP2A phosphatase to antagonize the Cdk1 phosphorylation .
	manualset3
86964	5	399551	5	NULL	NULL	0	NULL	PP2A phosphatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In Xenopus , Cdk1 phosphorylates Emi2 and both destabilizes and inactivates it , whereas Mos recruits PP2A phosphatase to antagonize the Cdk1 phosphorylation .
	manualset3
86965	6	399551	5	NULL	NULL	0	NULL	Cdk1 phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In Xenopus , Cdk1 phosphorylates Emi2 and both destabilizes and inactivates it , whereas Mos recruits PP2A phosphatase to antagonize the Cdk1 phosphorylation .
	manualset3
86966	1	399552	5	NULL	NULL	0	NULL	B-Myb	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In accordance , B-Myb also elevates endogenous A ( 2B ) AR mRNA and receptor activity , and this activity decreases cell proliferation .
	manualset3
86967	2	399552	5	NULL	NULL	0	NULL	endogenous A ( 2B ) AR mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In accordance , B-Myb also elevates endogenous A ( 2B ) AR mRNA and receptor activity , and this activity decreases cell proliferation .
	manualset3
86968	3	399552	5	NULL	NULL	0	NULL	receptor activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In accordance , B-Myb also elevates endogenous A ( 2B ) AR mRNA and receptor activity , and this activity decreases cell proliferation .
	manualset3
86969	4	399552	5	NULL	NULL	0	NULL	activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In accordance , B-Myb also elevates endogenous A ( 2B ) AR mRNA and receptor activity , and this activity decreases cell proliferation .
	manualset3
86970	5	399552	5	NULL	NULL	0	NULL	cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In accordance , B-Myb also elevates endogenous A ( 2B ) AR mRNA and receptor activity , and this activity decreases cell proliferation .
	manualset3
86971	1	399553	5	NULL	NULL	0	NULL	age-associated telomere attrition rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In accordance , the age-associated telomere attrition rate was more prominent in families with members displaying longer telomeres at a young age ( r = -0.691 , P & lt ; 0.001 ) .
	manualset3
86972	2	399553	5	NULL	NULL	0	NULL	families	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In accordance , the age-associated telomere attrition rate was more prominent in families with members displaying longer telomeres at a young age ( r = -0.691 , P & lt ; 0.001 ) .
	manualset3
86973	3	399553	5	NULL	NULL	0	NULL	members	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In accordance , the age-associated telomere attrition rate was more prominent in families with members displaying longer telomeres at a young age ( r = -0.691 , P & lt ; 0.001 ) .
	manualset3
86974	4	399553	5	NULL	NULL	0	NULL	telomeres	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	In accordance , the age-associated telomere attrition rate was more prominent in families with members displaying longer telomeres at a young age ( r = -0.691 , P & lt ; 0.001 ) .
	manualset3
86975	5	399553	5	NULL	NULL	0	NULL	young age	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In accordance , the age-associated telomere attrition rate was more prominent in families with members displaying longer telomeres at a young age ( r = -0.691 , P & lt ; 0.001 ) .
	manualset3
86976	6	399553	5	NULL	NULL	0	NULL	r = -0.691 , P & lt ; 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In accordance , the age-associated telomere attrition rate was more prominent in families with members displaying longer telomeres at a young age ( r = -0.691 , P & lt ; 0.001 ) .
	manualset3
86981	1	399555	5	NULL	NULL	NULL	NULL	determinations of phospholipase activity	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In agreement , determinations of phospholipase activity disclosed the presence of a phospholipase A2 in the fluid phase of synovial effusions .
	manualset3
86983	2	399555	5	NULL	NULL	NULL	NULL	phospholipase A2	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In agreement , determinations of phospholipase activity disclosed the presence of a phospholipase A2 in the fluid phase of synovial effusions .
	manualset3
86984	3	399555	5	NULL	NULL	NULL	NULL	fluid phase of synovial effusions	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In agreement , determinations of phospholipase activity disclosed the presence of a phospholipase A2 in the fluid phase of synovial effusions .
	manualset3
86985	1	399556	5	NULL	NULL	0	NULL	cardiomyocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In cardiomyocytes , Gq activates only one splice variant of one subtype of phospholipase Cbeta , specifically phospholipase Cbeta1b ( PLCbeta1b ) and PLCbeta1b is responsible for Gq mediated hypertrophic and apoptotic responses .
	manualset3
86986	2	399556	5	NULL	NULL	NULL	NULL	Gq	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In cardiomyocytes , Gq activates only one splice variant of one subtype of phospholipase Cbeta , specifically phospholipase Cbeta1b ( PLCbeta1b ) and PLCbeta1b is responsible for Gq mediated hypertrophic and apoptotic responses .
	manualset3
86987	3	399556	5	NULL	NULL	NULL	NULL	splice variant of one subtype of phospholipase Cbeta	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In cardiomyocytes , Gq activates only one splice variant of one subtype of phospholipase Cbeta , specifically phospholipase Cbeta1b ( PLCbeta1b ) and PLCbeta1b is responsible for Gq mediated hypertrophic and apoptotic responses .
	manualset3
86988	4	399556	5	NULL	NULL	0	NULL	phospholipase Cbeta1b ( PLCbeta1b )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In cardiomyocytes , Gq activates only one splice variant of one subtype of phospholipase Cbeta , specifically phospholipase Cbeta1b ( PLCbeta1b ) and PLCbeta1b is responsible for Gq mediated hypertrophic and apoptotic responses .
	manualset3
86989	5	399556	5	NULL	NULL	0	NULL	PLCbeta1b	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In cardiomyocytes , Gq activates only one splice variant of one subtype of phospholipase Cbeta , specifically phospholipase Cbeta1b ( PLCbeta1b ) and PLCbeta1b is responsible for Gq mediated hypertrophic and apoptotic responses .
	manualset3
86990	6	399556	5	NULL	NULL	NULL	NULL	Gq mediated hypertrophic responses	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In cardiomyocytes , Gq activates only one splice variant of one subtype of phospholipase Cbeta , specifically phospholipase Cbeta1b ( PLCbeta1b ) and PLCbeta1b is responsible for Gq mediated hypertrophic and apoptotic responses .
	manualset3
86991	7	399556	5	NULL	NULL	0	NULL	Gq mediated apoptotic responses	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In cardiomyocytes , Gq activates only one splice variant of one subtype of phospholipase Cbeta , specifically phospholipase Cbeta1b ( PLCbeta1b ) and PLCbeta1b is responsible for Gq mediated hypertrophic and apoptotic responses .
	manualset3
86992	1	399557	5	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In children , consumption of soy-based formulas and soy milk can lead to high levels of exposure to phytoestrogens with only limited data available concerning potential benefits or adverse effects .
	manualset3
86993	2	399557	5	NULL	NULL	0	NULL	consumption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In children , consumption of soy-based formulas and soy milk can lead to high levels of exposure to phytoestrogens with only limited data available concerning potential benefits or adverse effects .
	manualset3
86994	3	399557	5	NULL	NULL	0	NULL	soy-based formulas	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	In children , consumption of soy-based formulas and soy milk can lead to high levels of exposure to phytoestrogens with only limited data available concerning potential benefits or adverse effects .
	manualset3
86995	4	399557	5	NULL	NULL	0	NULL	soy milk	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	In children , consumption of soy-based formulas and soy milk can lead to high levels of exposure to phytoestrogens with only limited data available concerning potential benefits or adverse effects .
	manualset3
86996	5	399557	5	NULL	NULL	NULL	NULL	high levels of exposure to phytoestrogens	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In children , consumption of soy-based formulas and soy milk can lead to high levels of exposure to phytoestrogens with only limited data available concerning potential benefits or adverse effects .
	manualset3
86997	6	399557	5	NULL	NULL	0	NULL	limited data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In children , consumption of soy-based formulas and soy milk can lead to high levels of exposure to phytoestrogens with only limited data available concerning potential benefits or adverse effects .
	manualset3
86998	7	399557	5	NULL	NULL	0	NULL	potential benefits or adverse effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In children , consumption of soy-based formulas and soy milk can lead to high levels of exposure to phytoestrogens with only limited data available concerning potential benefits or adverse effects .
	manualset3
87103	1	399558	5	NULL	NULL	0	NULL	antagonists	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In combination , these antagonists almost completely inhibited contraction to both agents .
	manualset3
87105	2	399558	5	NULL	NULL	0	NULL	contraction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In combination , these antagonists almost completely inhibited contraction to both agents .
	manualset3
87107	3	399558	5	NULL	NULL	0	NULL	agents	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In combination , these antagonists almost completely inhibited contraction to both agents .
	manualset3
87109	1	399559	5	NULL	NULL	0	NULL	smaller plasma forms	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison , smaller plasma forms circulating in blood bind platelets only under high fluid shear stress or induced by modulators .
	manualset3
87110	2	399559	5	NULL	NULL	0	NULL	blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison , smaller plasma forms circulating in blood bind platelets only under high fluid shear stress or induced by modulators .
	manualset3
87111	3	399559	5	NULL	NULL	0	NULL	platelets	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison , smaller plasma forms circulating in blood bind platelets only under high fluid shear stress or induced by modulators .
	manualset3
87112	4	399559	5	NULL	NULL	0	NULL	high fluid shear stress	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison , smaller plasma forms circulating in blood bind platelets only under high fluid shear stress or induced by modulators .
	manualset3
87113	5	399559	5	NULL	NULL	0	NULL	modulators	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison , smaller plasma forms circulating in blood bind platelets only under high fluid shear stress or induced by modulators .
	manualset3
87115	1	399560	5	NULL	NULL	0	NULL	CCK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , CCK is a potential candidate as a physiological factor regulating insulin secretion in sheep .
	manualset3
87116	2	399560	5	NULL	NULL	0	NULL	potential candidate	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , CCK is a potential candidate as a physiological factor regulating insulin secretion in sheep .
	manualset3
87117	3	399560	5	NULL	NULL	0	NULL	physiological factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , CCK is a potential candidate as a physiological factor regulating insulin secretion in sheep .
	manualset3
87121	4	399560	5	NULL	NULL	0	NULL	insulin secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , CCK is a potential candidate as a physiological factor regulating insulin secretion in sheep .
	manualset3
87122	5	399560	5	NULL	NULL	0	NULL	sheep	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , CCK is a potential candidate as a physiological factor regulating insulin secretion in sheep .
	manualset3
87123	1	399561	5	NULL	NULL	0	NULL	CHB patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , CHB patients with genotype B , G1896A , and A1762T/G1764A had a higher tendency to develop liver failure than patients with genotype C. Therefore , HBV genotyping and detecting G1896A and A1762T/G1764A mutations might have important clinical implications as predictive risk factors for hepatitis B-related acute-on-chronic liver failure .
	manualset3
87127	2	399561	5	NULL	NULL	0	NULL	genotype B , G1896A , and A1762T/G1764A	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , CHB patients with genotype B , G1896A , and A1762T/G1764A had a higher tendency to develop liver failure than patients with genotype C. Therefore , HBV genotyping and detecting G1896A and A1762T/G1764A mutations might have important clinical implications as predictive risk factors for hepatitis B-related acute-on-chronic liver failure .
	manualset3
87128	3	399561	5	NULL	NULL	0	NULL	liver failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , CHB patients with genotype B , G1896A , and A1762T/G1764A had a higher tendency to develop liver failure than patients with genotype C. Therefore , HBV genotyping and detecting G1896A and A1762T/G1764A mutations might have important clinical implications as predictive risk factors for hepatitis B-related acute-on-chronic liver failure .
	manualset3
87129	4	399561	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , CHB patients with genotype B , G1896A , and A1762T/G1764A had a higher tendency to develop liver failure than patients with genotype C. Therefore , HBV genotyping and detecting G1896A and A1762T/G1764A mutations might have important clinical implications as predictive risk factors for hepatitis B-related acute-on-chronic liver failure .
	manualset3
87130	5	399561	5	NULL	NULL	0	NULL	genotype C	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , CHB patients with genotype B , G1896A , and A1762T/G1764A had a higher tendency to develop liver failure than patients with genotype C. Therefore , HBV genotyping and detecting G1896A and A1762T/G1764A mutations might have important clinical implications as predictive risk factors for hepatitis B-related acute-on-chronic liver failure .
	manualset3
87133	6	399561	5	NULL	NULL	0	NULL	HBV genotyping	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , CHB patients with genotype B , G1896A , and A1762T/G1764A had a higher tendency to develop liver failure than patients with genotype C. Therefore , HBV genotyping and detecting G1896A and A1762T/G1764A mutations might have important clinical implications as predictive risk factors for hepatitis B-related acute-on-chronic liver failure .
	manualset3
87134	7	399561	5	NULL	NULL	0	NULL	G1896A and A1762T/G1764A mutations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , CHB patients with genotype B , G1896A , and A1762T/G1764A had a higher tendency to develop liver failure than patients with genotype C. Therefore , HBV genotyping and detecting G1896A and A1762T/G1764A mutations might have important clinical implications as predictive risk factors for hepatitis B-related acute-on-chronic liver failure .
	manualset3
87135	8	399561	5	NULL	NULL	0	NULL	important clinical implications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , CHB patients with genotype B , G1896A , and A1762T/G1764A had a higher tendency to develop liver failure than patients with genotype C. Therefore , HBV genotyping and detecting G1896A and A1762T/G1764A mutations might have important clinical implications as predictive risk factors for hepatitis B-related acute-on-chronic liver failure .
	manualset3
87136	9	399561	5	NULL	NULL	NULL	NULL	predictive risk factors	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion , CHB patients with genotype B , G1896A , and A1762T/G1764A had a higher tendency to develop liver failure than patients with genotype C. Therefore , HBV genotyping and detecting G1896A and A1762T/G1764A mutations might have important clinical implications as predictive risk factors for hepatitis B-related acute-on-chronic liver failure .
	manualset3
87137	10	399561	5	NULL	NULL	0	NULL	hepatitis B-related acute-on-chronic liver failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , CHB patients with genotype B , G1896A , and A1762T/G1764A had a higher tendency to develop liver failure than patients with genotype C. Therefore , HBV genotyping and detecting G1896A and A1762T/G1764A mutations might have important clinical implications as predictive risk factors for hepatitis B-related acute-on-chronic liver failure .
	manualset3
87139	2	399562	5	NULL	NULL	0	NULL	Candida albicans ATCC 90028	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , Candida albicans ATCC 90028 possesses an alternative electron transfer chain and alternative oxidase , both absent in animal cells .
	manualset3
87140	3	399562	5	NULL	NULL	0	NULL	alternative electron transfer chain	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , Candida albicans ATCC 90028 possesses an alternative electron transfer chain and alternative oxidase , both absent in animal cells .
	manualset3
87141	4	399562	5	NULL	NULL	0	NULL	alternative oxidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , Candida albicans ATCC 90028 possesses an alternative electron transfer chain and alternative oxidase , both absent in animal cells .
	manualset3
87142	5	399562	5	NULL	NULL	0	NULL	animal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , Candida albicans ATCC 90028 possesses an alternative electron transfer chain and alternative oxidase , both absent in animal cells .
	manualset3
87143	1	399563	5	NULL	NULL	0	NULL	structure-based design	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Towards structure-based design of novel inhibitors for V-ATPase ) .
	manualset3
87144	2	399563	5	NULL	NULL	0	NULL	novel inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Towards structure-based design of novel inhibitors for V-ATPase ) .
	manualset3
87145	3	399563	5	NULL	NULL	0	NULL	V-ATPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Towards structure-based design of novel inhibitors for V-ATPase ) .
	manualset3
87147	1	399564	5	NULL	NULL	NULL	NULL	ET-1 secretion	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion , ET-1 secretion is increased by Prepro-ET-1 overexpression .
	manualset3
87148	2	399564	5	NULL	NULL	NULL	NULL	Prepro-ET-1 overexpression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion , ET-1 secretion is increased by Prepro-ET-1 overexpression .
	manualset3
87150	2	399565	5	NULL	NULL	0	NULL	HDAC activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , HDAC activity is not essential for the strong transcriptional repressor activity mediated by the KRAB domain of Kox1 in particular and , presumably , by KRAB domains in general .
	manualset3
87151	3	399565	5	NULL	NULL	0	NULL	strong transcriptional repressor activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , HDAC activity is not essential for the strong transcriptional repressor activity mediated by the KRAB domain of Kox1 in particular and , presumably , by KRAB domains in general .
	manualset3
87152	4	399565	5	NULL	NULL	0	NULL	KRAB domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , HDAC activity is not essential for the strong transcriptional repressor activity mediated by the KRAB domain of Kox1 in particular and , presumably , by KRAB domains in general .
	manualset3
87153	5	399565	5	NULL	NULL	0	NULL	Kox1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , HDAC activity is not essential for the strong transcriptional repressor activity mediated by the KRAB domain of Kox1 in particular and , presumably , by KRAB domains in general .
	manualset3
87154	6	399565	5	NULL	NULL	0	NULL	KRAB domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , HDAC activity is not essential for the strong transcriptional repressor activity mediated by the KRAB domain of Kox1 in particular and , presumably , by KRAB domains in general .
	manualset3
87156	2	399566	5	NULL	NULL	0	NULL	JAK2 exon 12 mutation analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , JAK2 exon 12 mutation analysis contributes to diagnostics in polycythemia vera or erythrocytosis .
	manualset3
87157	3	399566	5	NULL	NULL	0	NULL	diagnostics	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , JAK2 exon 12 mutation analysis contributes to diagnostics in polycythemia vera or erythrocytosis .
	manualset3
87158	4	399566	5	NULL	NULL	0	NULL	polycythemia vera or erythrocytosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , JAK2 exon 12 mutation analysis contributes to diagnostics in polycythemia vera or erythrocytosis .
	manualset3
87160	2	399567	5	NULL	NULL	0	NULL	MVs	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , MVs released from MSCs were found to exert a pro-survival effect on renal cells in vitro and in vivo , suggesting that MVs may contribute to renal protection conferred by MSCs .
	manualset3
87161	3	399567	5	NULL	NULL	0	NULL	MSCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , MVs released from MSCs were found to exert a pro-survival effect on renal cells in vitro and in vivo , suggesting that MVs may contribute to renal protection conferred by MSCs .
	manualset3
87162	4	399567	5	NULL	NULL	0	NULL	pro-survival effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , MVs released from MSCs were found to exert a pro-survival effect on renal cells in vitro and in vivo , suggesting that MVs may contribute to renal protection conferred by MSCs .
	manualset3
87163	5	399567	5	NULL	NULL	0	NULL	renal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , MVs released from MSCs were found to exert a pro-survival effect on renal cells in vitro and in vivo , suggesting that MVs may contribute to renal protection conferred by MSCs .
	manualset3
87164	6	399567	5	NULL	NULL	0	NULL	MVs	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , MVs released from MSCs were found to exert a pro-survival effect on renal cells in vitro and in vivo , suggesting that MVs may contribute to renal protection conferred by MSCs .
	manualset3
87165	7	399567	5	NULL	NULL	0	NULL	renal protection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , MVs released from MSCs were found to exert a pro-survival effect on renal cells in vitro and in vivo , suggesting that MVs may contribute to renal protection conferred by MSCs .
	manualset3
87166	8	399567	5	NULL	NULL	0	NULL	MSCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , MVs released from MSCs were found to exert a pro-survival effect on renal cells in vitro and in vivo , suggesting that MVs may contribute to renal protection conferred by MSCs .
	manualset3
87168	2	399568	5	NULL	NULL	0	NULL	SK	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , SK & F L-94901 discriminates hepatic cells and pituitary cells at the nuclear transport process .
	manualset3
87169	3	399568	5	NULL	NULL	0	NULL	F L-94901	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , SK & F L-94901 discriminates hepatic cells and pituitary cells at the nuclear transport process .
	manualset3
87170	4	399568	5	NULL	NULL	0	NULL	hepatic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , SK & F L-94901 discriminates hepatic cells and pituitary cells at the nuclear transport process .
	manualset3
87171	5	399568	5	NULL	NULL	0	NULL	pituitary cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , SK & F L-94901 discriminates hepatic cells and pituitary cells at the nuclear transport process .
	manualset3
87172	6	399568	5	NULL	NULL	0	NULL	nuclear transport process	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , SK & F L-94901 discriminates hepatic cells and pituitary cells at the nuclear transport process .
	manualset3
87174	2	399569	5	NULL	NULL	NULL	NULL	TiO ( 2 ) nanotubes	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion , TiO ( 2 ) nanotubes can modulate bone formation events at the bone-implant interface as to reach favorable molecular response and osseointegration ; in addition , the diameters of nanotubes can be precisely controlled in order to obtain better bone formation .
	manualset3
87175	3	399569	5	NULL	NULL	0	NULL	bone formation events	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , TiO ( 2 ) nanotubes can modulate bone formation events at the bone-implant interface as to reach favorable molecular response and osseointegration ; in addition , the diameters of nanotubes can be precisely controlled in order to obtain better bone formation .
	manualset3
87176	4	399569	5	NULL	NULL	0	NULL	bone-implant interface	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , TiO ( 2 ) nanotubes can modulate bone formation events at the bone-implant interface as to reach favorable molecular response and osseointegration ; in addition , the diameters of nanotubes can be precisely controlled in order to obtain better bone formation .
	manualset3
87177	5	399569	5	NULL	NULL	0	NULL	favorable molecular response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , TiO ( 2 ) nanotubes can modulate bone formation events at the bone-implant interface as to reach favorable molecular response and osseointegration ; in addition , the diameters of nanotubes can be precisely controlled in order to obtain better bone formation .
	manualset3
87178	6	399569	5	NULL	NULL	0	NULL	osseointegration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , TiO ( 2 ) nanotubes can modulate bone formation events at the bone-implant interface as to reach favorable molecular response and osseointegration ; in addition , the diameters of nanotubes can be precisely controlled in order to obtain better bone formation .
	manualset3
87180	7	399569	5	NULL	NULL	0	NULL	diameters	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , TiO ( 2 ) nanotubes can modulate bone formation events at the bone-implant interface as to reach favorable molecular response and osseointegration ; in addition , the diameters of nanotubes can be precisely controlled in order to obtain better bone formation .
	manualset3
87181	8	399569	5	NULL	NULL	0	NULL	nanotubes	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , TiO ( 2 ) nanotubes can modulate bone formation events at the bone-implant interface as to reach favorable molecular response and osseointegration ; in addition , the diameters of nanotubes can be precisely controlled in order to obtain better bone formation .
	manualset3
87182	9	399569	5	NULL	NULL	0	NULL	bone formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , TiO ( 2 ) nanotubes can modulate bone formation events at the bone-implant interface as to reach favorable molecular response and osseointegration ; in addition , the diameters of nanotubes can be precisely controlled in order to obtain better bone formation .
	manualset3
87186	2	399570	5	NULL	NULL	0	NULL	12-week dietary fat modification	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , a 12-week dietary fat modification did not affect the investigated markers of oxidative stress and inflammation among subjects with the MetS in the LIPGENE study .
	manualset3
87188	3	399570	5	NULL	NULL	0	NULL	markers of oxidative stress and inflammation	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , a 12-week dietary fat modification did not affect the investigated markers of oxidative stress and inflammation among subjects with the MetS in the LIPGENE study .
	manualset3
87191	4	399570	5	NULL	NULL	0	NULL	subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , a 12-week dietary fat modification did not affect the investigated markers of oxidative stress and inflammation among subjects with the MetS in the LIPGENE study .
	manualset3
87192	5	399570	5	NULL	NULL	0	NULL	MetS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , a 12-week dietary fat modification did not affect the investigated markers of oxidative stress and inflammation among subjects with the MetS in the LIPGENE study .
	manualset3
87193	6	399570	5	NULL	NULL	0	NULL	LIPGENE study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , a 12-week dietary fat modification did not affect the investigated markers of oxidative stress and inflammation among subjects with the MetS in the LIPGENE study .
	manualset3
87197	2	399571	5	NULL	NULL	0	NULL	Roux-en-Y gastric bypass	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , after Roux-en-Y gastric bypass , energy economy hampers the weight loss process , probably through a low fat oxidation rate .
	manualset3
87198	3	399571	5	NULL	NULL	0	NULL	energy economy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , after Roux-en-Y gastric bypass , energy economy hampers the weight loss process , probably through a low fat oxidation rate .
	manualset3
87199	4	399571	5	NULL	NULL	0	NULL	weight loss process	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , after Roux-en-Y gastric bypass , energy economy hampers the weight loss process , probably through a low fat oxidation rate .
	manualset3
87201	5	399571	5	NULL	NULL	0	NULL	low fat oxidation rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , after Roux-en-Y gastric bypass , energy economy hampers the weight loss process , probably through a low fat oxidation rate .
	manualset3
87206	2	399572	5	NULL	NULL	0	NULL	detailed mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , although the detailed mechanism for the anti-tumor activity of the P. cocos beta-glucan still needs further investigation , this study provides preliminary insights into its mode of action and perspectives of its development as a water-soluble anti-tumor agent .
	manualset3
87207	3	399572	5	NULL	NULL	0	NULL	anti-tumor activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , although the detailed mechanism for the anti-tumor activity of the P. cocos beta-glucan still needs further investigation , this study provides preliminary insights into its mode of action and perspectives of its development as a water-soluble anti-tumor agent .
	manualset3
87210	4	399572	5	NULL	NULL	0	NULL	P. cocos beta-glucan	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , although the detailed mechanism for the anti-tumor activity of the P. cocos beta-glucan still needs further investigation , this study provides preliminary insights into its mode of action and perspectives of its development as a water-soluble anti-tumor agent .
	manualset3
87211	5	399572	5	NULL	NULL	0	NULL	investigation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , although the detailed mechanism for the anti-tumor activity of the P. cocos beta-glucan still needs further investigation , this study provides preliminary insights into its mode of action and perspectives of its development as a water-soluble anti-tumor agent .
	manualset3
87212	6	399572	5	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , although the detailed mechanism for the anti-tumor activity of the P. cocos beta-glucan still needs further investigation , this study provides preliminary insights into its mode of action and perspectives of its development as a water-soluble anti-tumor agent .
	manualset3
87214	7	399572	5	NULL	NULL	0	NULL	preliminary insights	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , although the detailed mechanism for the anti-tumor activity of the P. cocos beta-glucan still needs further investigation , this study provides preliminary insights into its mode of action and perspectives of its development as a water-soluble anti-tumor agent .
	manualset3
87215	8	399572	5	NULL	NULL	0	NULL	mode of action	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , although the detailed mechanism for the anti-tumor activity of the P. cocos beta-glucan still needs further investigation , this study provides preliminary insights into its mode of action and perspectives of its development as a water-soluble anti-tumor agent .
	manualset3
87218	9	399572	5	NULL	NULL	0	NULL	water-soluble anti-tumor agent	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , although the detailed mechanism for the anti-tumor activity of the P. cocos beta-glucan still needs further investigation , this study provides preliminary insights into its mode of action and perspectives of its development as a water-soluble anti-tumor agent .
	manualset3
87222	2	399573	5	NULL	NULL	0	NULL	anaplerosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , anaplerosis that enhances the supply and utilization of alpha-ketoglutarate in the tricarboxylic acid cycle appears to play an essential role in the generation of TDP .
	manualset3
87224	3	399573	5	NULL	NULL	0	NULL	supply and utilization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , anaplerosis that enhances the supply and utilization of alpha-ketoglutarate in the tricarboxylic acid cycle appears to play an essential role in the generation of TDP .
	manualset3
87226	4	399573	5	NULL	NULL	0	NULL	alpha-ketoglutarate	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , anaplerosis that enhances the supply and utilization of alpha-ketoglutarate in the tricarboxylic acid cycle appears to play an essential role in the generation of TDP .
	manualset3
87227	5	399573	5	NULL	NULL	0	NULL	tricarboxylic acid cycle	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , anaplerosis that enhances the supply and utilization of alpha-ketoglutarate in the tricarboxylic acid cycle appears to play an essential role in the generation of TDP .
	manualset3
87228	6	399573	5	NULL	NULL	0	NULL	generation of TDP	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , anaplerosis that enhances the supply and utilization of alpha-ketoglutarate in the tricarboxylic acid cycle appears to play an essential role in the generation of TDP .
	manualset3
87229	1	399574	5	NULL	NULL	0	NULL	Toxic reaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Toxic reaction to bupivacaine ) .
	manualset3
87230	2	399574	5	NULL	NULL	0	NULL	bupivacaine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Toxic reaction to bupivacaine ) .
	manualset3
87235	2	399575	5	NULL	NULL	0	NULL	antimelanoma MoAb	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , antimelanoma MoAb was of little help in radioimaging and stating this disease .
	manualset3
87238	3	399575	5	NULL	NULL	0	NULL	radioimaging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , antimelanoma MoAb was of little help in radioimaging and stating this disease .
	manualset3
87239	4	399575	5	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , antimelanoma MoAb was of little help in radioimaging and stating this disease .
	manualset3
87241	2	399576	5	NULL	NULL	0	NULL	cartilage	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , cartilage is an available , costless , reliable and technically easy to use graft material for functional reconstructions of the ossicular chain .
	manualset3
87242	3	399576	5	NULL	NULL	0	NULL	graft material	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , cartilage is an available , costless , reliable and technically easy to use graft material for functional reconstructions of the ossicular chain .
	manualset3
87243	4	399576	5	NULL	NULL	0	NULL	functional reconstructions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , cartilage is an available , costless , reliable and technically easy to use graft material for functional reconstructions of the ossicular chain .
	manualset3
87244	5	399576	5	NULL	NULL	0	NULL	ossicular chain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , cartilage is an available , costless , reliable and technically easy to use graft material for functional reconstructions of the ossicular chain .
	manualset3
87246	2	399577	5	NULL	NULL	NULL	NULL	claudin-6 immunohistochemistry	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion , claudin-6 immunohistochemistry is of limited sensitivity and specificity for the diagnosis of AT/RT and does not correlate with clinical behavior .
	manualset3
87247	3	399577	5	NULL	NULL	0	NULL	limited sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , claudin-6 immunohistochemistry is of limited sensitivity and specificity for the diagnosis of AT/RT and does not correlate with clinical behavior .
	manualset3
87248	4	399577	5	NULL	NULL	0	NULL	specificity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , claudin-6 immunohistochemistry is of limited sensitivity and specificity for the diagnosis of AT/RT and does not correlate with clinical behavior .
	manualset3
87249	5	399577	5	NULL	NULL	0	NULL	 diagnosis of AT/RT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , claudin-6 immunohistochemistry is of limited sensitivity and specificity for the diagnosis of AT/RT and does not correlate with clinical behavior .
	manualset3
87250	6	399577	5	NULL	NULL	0	NULL	clinical behavior	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , claudin-6 immunohistochemistry is of limited sensitivity and specificity for the diagnosis of AT/RT and does not correlate with clinical behavior .
	manualset3
87252	2	399578	5	NULL	NULL	0	NULL	consumption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , consumption of drinking water , especially well water , with high nitrate levels can imply a genotoxic risk for humans as indicated by increased HPRT variant frequencies and by endogenous formation of carcinogenic N-nitroso compounds from nitrate-derived nitrite .
	manualset3
87253	3	399578	5	NULL	NULL	0	NULL	drinking water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , consumption of drinking water , especially well water , with high nitrate levels can imply a genotoxic risk for humans as indicated by increased HPRT variant frequencies and by endogenous formation of carcinogenic N-nitroso compounds from nitrate-derived nitrite .
	manualset3
87254	4	399578	5	NULL	NULL	0	NULL	well water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , consumption of drinking water , especially well water , with high nitrate levels can imply a genotoxic risk for humans as indicated by increased HPRT variant frequencies and by endogenous formation of carcinogenic N-nitroso compounds from nitrate-derived nitrite .
	manualset3
87255	5	399578	5	NULL	NULL	0	NULL	high nitrate levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , consumption of drinking water , especially well water , with high nitrate levels can imply a genotoxic risk for humans as indicated by increased HPRT variant frequencies and by endogenous formation of carcinogenic N-nitroso compounds from nitrate-derived nitrite .
	manualset3
87256	6	399578	5	NULL	NULL	0	NULL	genotoxic risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , consumption of drinking water , especially well water , with high nitrate levels can imply a genotoxic risk for humans as indicated by increased HPRT variant frequencies and by endogenous formation of carcinogenic N-nitroso compounds from nitrate-derived nitrite .
	manualset3
87257	7	399578	5	NULL	NULL	0	NULL	humans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , consumption of drinking water , especially well water , with high nitrate levels can imply a genotoxic risk for humans as indicated by increased HPRT variant frequencies and by endogenous formation of carcinogenic N-nitroso compounds from nitrate-derived nitrite .
	manualset3
87258	8	399578	5	NULL	NULL	0	NULL	increased HPRT variant frequencies	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , consumption of drinking water , especially well water , with high nitrate levels can imply a genotoxic risk for humans as indicated by increased HPRT variant frequencies and by endogenous formation of carcinogenic N-nitroso compounds from nitrate-derived nitrite .
	manualset3
87259	9	399578	5	NULL	NULL	0	NULL	endogenous formation of carcinogenic N-nitroso compounds from nitrate-derived nitrite	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , consumption of drinking water , especially well water , with high nitrate levels can imply a genotoxic risk for humans as indicated by increased HPRT variant frequencies and by endogenous formation of carcinogenic N-nitroso compounds from nitrate-derived nitrite .
	manualset3
87261	2	399579	5	NULL	NULL	0	NULL	higher risk profile	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , despite a higher risk profile , CPS allowed longer balloon inflations and higher PTCA success rates compared to IABP .
	manualset3
87263	3	399579	5	NULL	NULL	0	NULL	CPS	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , despite a higher risk profile , CPS allowed longer balloon inflations and higher PTCA success rates compared to IABP .
	manualset3
87265	4	399579	5	NULL	NULL	0	NULL	longer balloon inflations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , despite a higher risk profile , CPS allowed longer balloon inflations and higher PTCA success rates compared to IABP .
	manualset3
87266	5	399579	5	NULL	NULL	0	NULL	higher PTCA success rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , despite a higher risk profile , CPS allowed longer balloon inflations and higher PTCA success rates compared to IABP .
	manualset3
87269	6	399579	5	NULL	NULL	0	NULL	IABP	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , despite a higher risk profile , CPS allowed longer balloon inflations and higher PTCA success rates compared to IABP .
	manualset3
87271	2	399580	5	NULL	NULL	0	NULL	early controlled mobilization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , early controlled mobilization using a hinged wrist splint may optimize the recovery period while retaining the desired arc of motion that is set intraoperatively .
	manualset3
87272	3	399580	5	NULL	NULL	0	NULL	hinged wrist splint	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , early controlled mobilization using a hinged wrist splint may optimize the recovery period while retaining the desired arc of motion that is set intraoperatively .
	manualset3
87273	4	399580	5	NULL	NULL	0	NULL	recovery period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , early controlled mobilization using a hinged wrist splint may optimize the recovery period while retaining the desired arc of motion that is set intraoperatively .
	manualset3
87274	5	399580	5	NULL	NULL	0	NULL	desired arc of motion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , early controlled mobilization using a hinged wrist splint may optimize the recovery period while retaining the desired arc of motion that is set intraoperatively .
	manualset3
87536	3	399581	5	NULL	NULL	NULL	NULL	DENV exposure	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion , evidence for DENV exposure , presumably to DENV-2 , was identified in residents from Central Anatolian provinces of Ankara and Konya for the first time , however , seroreactivity detected against YFV could not be confirmed by PRNT .
	manualset3
87537	4	399581	5	NULL	NULL	0	NULL	DENV-2	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , evidence for DENV exposure , presumably to DENV-2 , was identified in residents from Central Anatolian provinces of Ankara and Konya for the first time , however , seroreactivity detected against YFV could not be confirmed by PRNT .
	manualset3
87538	5	399581	5	NULL	NULL	0	NULL	residents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , evidence for DENV exposure , presumably to DENV-2 , was identified in residents from Central Anatolian provinces of Ankara and Konya for the first time , however , seroreactivity detected against YFV could not be confirmed by PRNT .
	manualset3
87539	6	399581	5	NULL	NULL	0	NULL	Central Anatolian provinces of Ankara and Konya	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , evidence for DENV exposure , presumably to DENV-2 , was identified in residents from Central Anatolian provinces of Ankara and Konya for the first time , however , seroreactivity detected against YFV could not be confirmed by PRNT .
	manualset3
87540	7	399581	5	NULL	NULL	0	NULL	seroreactivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , evidence for DENV exposure , presumably to DENV-2 , was identified in residents from Central Anatolian provinces of Ankara and Konya for the first time , however , seroreactivity detected against YFV could not be confirmed by PRNT .
	manualset3
87541	8	399581	5	NULL	NULL	0	NULL	YFV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , evidence for DENV exposure , presumably to DENV-2 , was identified in residents from Central Anatolian provinces of Ankara and Konya for the first time , however , seroreactivity detected against YFV could not be confirmed by PRNT .
	manualset3
87542	9	399581	5	NULL	NULL	0	NULL	PRNT	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , evidence for DENV exposure , presumably to DENV-2 , was identified in residents from Central Anatolian provinces of Ankara and Konya for the first time , however , seroreactivity detected against YFV could not be confirmed by PRNT .
	manualset3
87544	2	399582	5	NULL	NULL	0	NULL	high concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , high concentration of porphyrin precursors had little impact on renal function .
	manualset3
87545	3	399582	5	NULL	NULL	0	NULL	porphyrin precursors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , high concentration of porphyrin precursors had little impact on renal function .
	manualset3
87546	4	399582	5	NULL	NULL	0	NULL	renal function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , high concentration of porphyrin precursors had little impact on renal function .
	manualset3
87547	1	399583	5	NULL	NULL	0	NULL	Toxicity standardization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Toxicity and sanitary standardization of melamine cyanurate ( experimental data ) ) .
	manualset3
87548	3	399583	5	NULL	NULL	NULL	NULL	melamine cyanurate	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Toxicity and sanitary standardization of melamine cyanurate ( experimental data ) ) .
	manualset3
87549	4	399583	5	NULL	NULL	0	NULL	experimental data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Toxicity and sanitary standardization of melamine cyanurate ( experimental data ) ) .
	manualset3
87550	2	399583	5	NULL	NULL	0	NULL	sanitary standardization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Toxicity and sanitary standardization of melamine cyanurate ( experimental data ) ) .
	manualset3
87552	2	399584	5	NULL	NULL	0	NULL	tube	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , inserting the tube from the apex could shorten the treatment period .
	manualset3
87553	3	399584	5	NULL	NULL	0	NULL	apex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , inserting the tube from the apex could shorten the treatment period .
	manualset3
87554	4	399584	5	NULL	NULL	0	NULL	treatment period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , inserting the tube from the apex could shorten the treatment period .
	manualset3
87556	2	399585	5	NULL	NULL	0	NULL	delivery vehicle	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , it is of critical importance that the delivery vehicle prevents extensive aggregation of hypericin before injection and assures an efficient transfer to serum lipoproteins upon injection .
	manualset3
87557	3	399585	5	NULL	NULL	NULL	NULL	extensive aggregation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion , it is of critical importance that the delivery vehicle prevents extensive aggregation of hypericin before injection and assures an efficient transfer to serum lipoproteins upon injection .
	manualset3
87558	4	399585	5	NULL	NULL	0	NULL	hypericin	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , it is of critical importance that the delivery vehicle prevents extensive aggregation of hypericin before injection and assures an efficient transfer to serum lipoproteins upon injection .
	manualset3
87559	5	399585	5	NULL	NULL	0	NULL	injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , it is of critical importance that the delivery vehicle prevents extensive aggregation of hypericin before injection and assures an efficient transfer to serum lipoproteins upon injection .
	manualset3
87560	6	399585	5	NULL	NULL	0	NULL	efficient transfer	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , it is of critical importance that the delivery vehicle prevents extensive aggregation of hypericin before injection and assures an efficient transfer to serum lipoproteins upon injection .
	manualset3
87561	7	399585	5	NULL	NULL	0	NULL	serum lipoproteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , it is of critical importance that the delivery vehicle prevents extensive aggregation of hypericin before injection and assures an efficient transfer to serum lipoproteins upon injection .
	manualset3
87562	8	399585	5	NULL	NULL	0	NULL	injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , it is of critical importance that the delivery vehicle prevents extensive aggregation of hypericin before injection and assures an efficient transfer to serum lipoproteins upon injection .
	manualset3
87564	2	399586	5	NULL	NULL	0	NULL	nicotine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , nicotine enhances the chemoatactiveness of VSMC .
	manualset3
87565	3	399586	5	NULL	NULL	0	NULL	chemoatactiveness	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , nicotine enhances the chemoatactiveness of VSMC .
	manualset3
87566	4	399586	5	NULL	NULL	0	NULL	VSMC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , nicotine enhances the chemoatactiveness of VSMC .
	manualset3
87568	2	399587	5	NULL	NULL	0	NULL	techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , none of the techniques evaluated in this study was effective in providing complete removal of filling material from the root canals .
	manualset3
87569	3	399587	5	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , none of the techniques evaluated in this study was effective in providing complete removal of filling material from the root canals .
	manualset3
87570	4	399587	5	NULL	NULL	0	NULL	complete removal of filling material	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , none of the techniques evaluated in this study was effective in providing complete removal of filling material from the root canals .
	manualset3
87571	5	399587	5	NULL	NULL	0	NULL	root canals	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , none of the techniques evaluated in this study was effective in providing complete removal of filling material from the root canals .
	manualset3
87573	2	399588	5	NULL	NULL	0	NULL	objective assessment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , objective assessment of cough is practical in infants , enabling the pattern of cough in illness and in health to be studied further .
	manualset3
87574	3	399588	5	NULL	NULL	0	NULL	cough	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , objective assessment of cough is practical in infants , enabling the pattern of cough in illness and in health to be studied further .
	manualset3
87575	4	399588	5	NULL	NULL	0	NULL	infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , objective assessment of cough is practical in infants , enabling the pattern of cough in illness and in health to be studied further .
	manualset3
87576	5	399588	5	NULL	NULL	0	NULL	cough	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , objective assessment of cough is practical in infants , enabling the pattern of cough in illness and in health to be studied further .
	manualset3
87577	6	399588	5	NULL	NULL	0	NULL	illness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , objective assessment of cough is practical in infants , enabling the pattern of cough in illness and in health to be studied further .
	manualset3
87578	7	399588	5	NULL	NULL	NULL	NULL	health	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion , objective assessment of cough is practical in infants , enabling the pattern of cough in illness and in health to be studied further .
	manualset3
87580	2	399589	5	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our data provide evidence that adiponectin is up-regulated in vivo and in vitro in human and rodent myotubes in response to inflammatory stimuli .
	manualset3
87581	3	399589	5	NULL	NULL	0	NULL	adiponectin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our data provide evidence that adiponectin is up-regulated in vivo and in vitro in human and rodent myotubes in response to inflammatory stimuli .
	manualset3
87585	4	399589	5	NULL	NULL	0	NULL	human	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our data provide evidence that adiponectin is up-regulated in vivo and in vitro in human and rodent myotubes in response to inflammatory stimuli .
	manualset3
87586	5	399589	5	NULL	NULL	0	NULL	rodent myotubes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our data provide evidence that adiponectin is up-regulated in vivo and in vitro in human and rodent myotubes in response to inflammatory stimuli .
	manualset3
87587	6	399589	5	NULL	NULL	0	NULL	inflammatory stimuli	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our data provide evidence that adiponectin is up-regulated in vivo and in vitro in human and rodent myotubes in response to inflammatory stimuli .
	manualset3
87589	2	399590	5	NULL	NULL	0	NULL	T. b. brucei invasion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our data show that T. b. brucei invasion of the brain is related to that of leukocytes and that minocycline can ameliorate the disease in trypanosome-infected mice .
	manualset3
87590	3	399590	5	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our data show that T. b. brucei invasion of the brain is related to that of leukocytes and that minocycline can ameliorate the disease in trypanosome-infected mice .
	manualset3
87591	4	399590	5	NULL	NULL	0	NULL	leukocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our data show that T. b. brucei invasion of the brain is related to that of leukocytes and that minocycline can ameliorate the disease in trypanosome-infected mice .
	manualset3
87592	5	399590	5	NULL	NULL	0	NULL	minocycline	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our data show that T. b. brucei invasion of the brain is related to that of leukocytes and that minocycline can ameliorate the disease in trypanosome-infected mice .
	manualset3
87593	6	399590	5	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our data show that T. b. brucei invasion of the brain is related to that of leukocytes and that minocycline can ameliorate the disease in trypanosome-infected mice .
	manualset3
87594	7	399590	5	NULL	NULL	0	NULL	trypanosome-infected mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our data show that T. b. brucei invasion of the brain is related to that of leukocytes and that minocycline can ameliorate the disease in trypanosome-infected mice .
	manualset3
87596	2	399591	5	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our data support a role for ER in lung ADCAs , proposing a role for ER in lungcarcinogenesis , especially among smokers .
	manualset3
87597	3	399591	5	NULL	NULL	0	NULL	ER	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our data support a role for ER in lung ADCAs , proposing a role for ER in lungcarcinogenesis , especially among smokers .
	manualset3
87598	4	399591	5	NULL	NULL	0	NULL	lung ADCAs	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our data support a role for ER in lung ADCAs , proposing a role for ER in lungcarcinogenesis , especially among smokers .
	manualset3
87599	5	399591	5	NULL	NULL	0	NULL	ER	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our data support a role for ER in lung ADCAs , proposing a role for ER in lungcarcinogenesis , especially among smokers .
	manualset3
87600	6	399591	5	NULL	NULL	NULL	NULL	lungcarcinogenesis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion , our data support a role for ER in lung ADCAs , proposing a role for ER in lungcarcinogenesis , especially among smokers .
	manualset3
87601	7	399591	5	NULL	NULL	0	NULL	smokers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our data support a role for ER in lung ADCAs , proposing a role for ER in lungcarcinogenesis , especially among smokers .
	manualset3
87604	1	399592	5	NULL	NULL	NULL	NULL	beta-adrenoceptor stimulation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion , our findings confirm that beta-adrenoceptor stimulation is one condition where there may be an increased role of I ( Ks ) in action potential repolarisation .
	manualset3
87605	2	399592	5	NULL	NULL	NULL	NULL	role	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion , our findings confirm that beta-adrenoceptor stimulation is one condition where there may be an increased role of I ( Ks ) in action potential repolarisation .
	manualset3
87606	3	399592	5	NULL	NULL	NULL	NULL	I ( Ks )	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion , our findings confirm that beta-adrenoceptor stimulation is one condition where there may be an increased role of I ( Ks ) in action potential repolarisation .
	manualset3
87607	4	399592	5	NULL	NULL	NULL	NULL	action potential repolarisation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion , our findings confirm that beta-adrenoceptor stimulation is one condition where there may be an increased role of I ( Ks ) in action potential repolarisation .
	manualset3
87610	3	399593	5	NULL	NULL	0	NULL	expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our findings indicate that expression of TGF-alpha gene and protein in normal blood eosinophils is differently regulated by GM-CSF and IL-3 .
	manualset3
87611	4	399593	5	NULL	NULL	0	NULL	TGF-alpha gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our findings indicate that expression of TGF-alpha gene and protein in normal blood eosinophils is differently regulated by GM-CSF and IL-3 .
	manualset3
87612	5	399593	5	NULL	NULL	0	NULL	TGF-alpha protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our findings indicate that expression of TGF-alpha gene and protein in normal blood eosinophils is differently regulated by GM-CSF and IL-3 .
	manualset3
87613	6	399593	5	NULL	NULL	0	NULL	normal blood eosinophils	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our findings indicate that expression of TGF-alpha gene and protein in normal blood eosinophils is differently regulated by GM-CSF and IL-3 .
	manualset3
87614	7	399593	5	NULL	NULL	0	NULL	GM-CSF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our findings indicate that expression of TGF-alpha gene and protein in normal blood eosinophils is differently regulated by GM-CSF and IL-3 .
	manualset3
87615	8	399593	5	NULL	NULL	0	NULL	IL-3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our findings indicate that expression of TGF-alpha gene and protein in normal blood eosinophils is differently regulated by GM-CSF and IL-3 .
	manualset3
87617	2	399594	5	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion , our results imply a molecular mechanism for SAHA-induced apoptosis in BV-173 cells , which involves decreased protein expression levels of Bcr-Abl , c-Myc and HDAC3 .
	manualset3
87618	3	399594	5	NULL	NULL	0	NULL	molecular mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our results imply a molecular mechanism for SAHA-induced apoptosis in BV-173 cells , which involves decreased protein expression levels of Bcr-Abl , c-Myc and HDAC3 .
	manualset3
87619	4	399594	5	NULL	NULL	0	NULL	SAHA-induced apoptosis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our results imply a molecular mechanism for SAHA-induced apoptosis in BV-173 cells , which involves decreased protein expression levels of Bcr-Abl , c-Myc and HDAC3 .
	manualset3
87620	5	399594	5	NULL	NULL	0	NULL	BV-173 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our results imply a molecular mechanism for SAHA-induced apoptosis in BV-173 cells , which involves decreased protein expression levels of Bcr-Abl , c-Myc and HDAC3 .
	manualset3
87621	6	399594	5	NULL	NULL	0	NULL	protein expression levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our results imply a molecular mechanism for SAHA-induced apoptosis in BV-173 cells , which involves decreased protein expression levels of Bcr-Abl , c-Myc and HDAC3 .
	manualset3
87622	7	399594	5	NULL	NULL	0	NULL	Bcr-Abl	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our results imply a molecular mechanism for SAHA-induced apoptosis in BV-173 cells , which involves decreased protein expression levels of Bcr-Abl , c-Myc and HDAC3 .
	manualset3
87623	8	399594	5	NULL	NULL	0	NULL	c-Myc	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our results imply a molecular mechanism for SAHA-induced apoptosis in BV-173 cells , which involves decreased protein expression levels of Bcr-Abl , c-Myc and HDAC3 .
	manualset3
87624	9	399594	5	NULL	NULL	0	NULL	HDAC3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our results imply a molecular mechanism for SAHA-induced apoptosis in BV-173 cells , which involves decreased protein expression levels of Bcr-Abl , c-Myc and HDAC3 .
	manualset3
87626	2	399595	5	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our results indicated that the knockdown of Cox-2 expression suppressed the proliferation and invasion of colorectal cancer cells both invitro and invivo .
	manualset3
87627	3	399595	5	NULL	NULL	0	NULL	 knockdown	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our results indicated that the knockdown of Cox-2 expression suppressed the proliferation and invasion of colorectal cancer cells both invitro and invivo .
	manualset3
87628	4	399595	5	NULL	NULL	0	NULL	Cox-2 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our results indicated that the knockdown of Cox-2 expression suppressed the proliferation and invasion of colorectal cancer cells both invitro and invivo .
	manualset3
87629	5	399595	5	NULL	NULL	0	NULL	proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our results indicated that the knockdown of Cox-2 expression suppressed the proliferation and invasion of colorectal cancer cells both invitro and invivo .
	manualset3
87630	6	399595	5	NULL	NULL	0	NULL	invasion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our results indicated that the knockdown of Cox-2 expression suppressed the proliferation and invasion of colorectal cancer cells both invitro and invivo .
	manualset3
87631	7	399595	5	NULL	NULL	0	NULL	colorectal cancer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , our results indicated that the knockdown of Cox-2 expression suppressed the proliferation and invasion of colorectal cancer cells both invitro and invivo .
	manualset3
87633	2	399596	5	NULL	NULL	0	NULL	oxidation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , oxidation of Trx1 and sustained Txnip expression in the lungs of newborn mice exposed to 85 % oxygen is likely to severely attenuate normal Trx1 function .
	manualset3
87634	3	399596	5	NULL	NULL	0	NULL	Trx1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , oxidation of Trx1 and sustained Txnip expression in the lungs of newborn mice exposed to 85 % oxygen is likely to severely attenuate normal Trx1 function .
	manualset3
87635	4	399596	5	NULL	NULL	0	NULL	sustained Txnip expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , oxidation of Trx1 and sustained Txnip expression in the lungs of newborn mice exposed to 85 % oxygen is likely to severely attenuate normal Trx1 function .
	manualset3
87636	5	399596	5	NULL	NULL	0	NULL	lungs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , oxidation of Trx1 and sustained Txnip expression in the lungs of newborn mice exposed to 85 % oxygen is likely to severely attenuate normal Trx1 function .
	manualset3
87637	6	399596	5	NULL	NULL	0	NULL	newborn mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , oxidation of Trx1 and sustained Txnip expression in the lungs of newborn mice exposed to 85 % oxygen is likely to severely attenuate normal Trx1 function .
	manualset3
87638	7	399596	5	NULL	NULL	NULL	NULL	85 % oxygen	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion , oxidation of Trx1 and sustained Txnip expression in the lungs of newborn mice exposed to 85 % oxygen is likely to severely attenuate normal Trx1 function .
	manualset3
87639	8	399596	5	NULL	NULL	0	NULL	normal Trx1 function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , oxidation of Trx1 and sustained Txnip expression in the lungs of newborn mice exposed to 85 % oxygen is likely to severely attenuate normal Trx1 function .
	manualset3
87641	2	399597	5	NULL	NULL	0	NULL	p38 MAPK-induced myocardial ischemic injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , p38 MAPK-induced myocardial ischemic injury is not modulated by MK2 .
	manualset3
87642	3	399597	5	NULL	NULL	0	NULL	MK2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , p38 MAPK-induced myocardial ischemic injury is not modulated by MK2 .
	manualset3
87647	2	399599	5	NULL	NULL	0	NULL	sera	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , sera from AIH-1 patients reacted with the amino acids in the sequence 33-37 ( PQDGS ) of the N-terminal of UGT1A6 .
	manualset3
87648	3	399599	5	NULL	NULL	0	NULL	AIH-1 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , sera from AIH-1 patients reacted with the amino acids in the sequence 33-37 ( PQDGS ) of the N-terminal of UGT1A6 .
	manualset3
87649	4	399599	5	NULL	NULL	0	NULL	amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , sera from AIH-1 patients reacted with the amino acids in the sequence 33-37 ( PQDGS ) of the N-terminal of UGT1A6 .
	manualset3
87650	5	399599	5	NULL	NULL	0	NULL	sequence 33-37 ( PQDGS )	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , sera from AIH-1 patients reacted with the amino acids in the sequence 33-37 ( PQDGS ) of the N-terminal of UGT1A6 .
	manualset3
87651	6	399599	5	NULL	NULL	0	NULL	N-terminal of UGT1A6	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , sera from AIH-1 patients reacted with the amino acids in the sequence 33-37 ( PQDGS ) of the N-terminal of UGT1A6 .
	manualset3
87658	2	399600	5	NULL	NULL	0	NULL	solid-state surface acidity measurement	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , solid-state surface acidity measurement of excipients and solid formulations using pH indicator probes as surrogates can be used to determine the ionization state of the drug and to predict the chemical stability profile of the drug in actual solid formulations .
	manualset3
87663	3	399600	5	NULL	NULL	0	NULL	excipients	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , solid-state surface acidity measurement of excipients and solid formulations using pH indicator probes as surrogates can be used to determine the ionization state of the drug and to predict the chemical stability profile of the drug in actual solid formulations .
	manualset3
87664	4	399600	5	NULL	NULL	NULL	NULL	solid formulations	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion , solid-state surface acidity measurement of excipients and solid formulations using pH indicator probes as surrogates can be used to determine the ionization state of the drug and to predict the chemical stability profile of the drug in actual solid formulations .
	manualset3
87665	5	399600	5	NULL	NULL	NULL	NULL	pH indicator probes	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion , solid-state surface acidity measurement of excipients and solid formulations using pH indicator probes as surrogates can be used to determine the ionization state of the drug and to predict the chemical stability profile of the drug in actual solid formulations .
	manualset3
87666	6	399600	5	NULL	NULL	NULL	NULL	surrogates	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion , solid-state surface acidity measurement of excipients and solid formulations using pH indicator probes as surrogates can be used to determine the ionization state of the drug and to predict the chemical stability profile of the drug in actual solid formulations .
	manualset3
87667	7	399600	5	NULL	NULL	0	NULL	drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , solid-state surface acidity measurement of excipients and solid formulations using pH indicator probes as surrogates can be used to determine the ionization state of the drug and to predict the chemical stability profile of the drug in actual solid formulations .
	manualset3
87668	8	399600	5	NULL	NULL	0	NULL	drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , solid-state surface acidity measurement of excipients and solid formulations using pH indicator probes as surrogates can be used to determine the ionization state of the drug and to predict the chemical stability profile of the drug in actual solid formulations .
	manualset3
87669	9	399600	5	NULL	NULL	NULL	NULL	actual solid formulations	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion , solid-state surface acidity measurement of excipients and solid formulations using pH indicator probes as surrogates can be used to determine the ionization state of the drug and to predict the chemical stability profile of the drug in actual solid formulations .
	manualset3
87671	2	399601	5	NULL	NULL	0	NULL	steroid saponins TTS-12 and TTS-15	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , steroid saponins TTS-12 and TTS-15 from Tribulus terrestris L. have significant in vitro antifungal activity against fluconazole-resistant fungi , especially TTS-12 also showed in vivo activity against fluconazole-resistant C. albicans .
	manualset3
87672	3	399601	5	NULL	NULL	0	NULL	Tribulus terrestris L.	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , steroid saponins TTS-12 and TTS-15 from Tribulus terrestris L. have significant in vitro antifungal activity against fluconazole-resistant fungi , especially TTS-12 also showed in vivo activity against fluconazole-resistant C. albicans .
	manualset3
87673	4	399601	5	NULL	NULL	0	NULL	in vitro antifungal activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , steroid saponins TTS-12 and TTS-15 from Tribulus terrestris L. have significant in vitro antifungal activity against fluconazole-resistant fungi , especially TTS-12 also showed in vivo activity against fluconazole-resistant C. albicans .
	manualset3
87674	5	399601	5	NULL	NULL	0	NULL	fluconazole-resistant fungi	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , steroid saponins TTS-12 and TTS-15 from Tribulus terrestris L. have significant in vitro antifungal activity against fluconazole-resistant fungi , especially TTS-12 also showed in vivo activity against fluconazole-resistant C. albicans .
	manualset3
87675	6	399601	5	NULL	NULL	0	NULL	TTS-12	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , steroid saponins TTS-12 and TTS-15 from Tribulus terrestris L. have significant in vitro antifungal activity against fluconazole-resistant fungi , especially TTS-12 also showed in vivo activity against fluconazole-resistant C. albicans .
	manualset3
87676	7	399601	5	NULL	NULL	0	NULL	in vivo activity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , steroid saponins TTS-12 and TTS-15 from Tribulus terrestris L. have significant in vitro antifungal activity against fluconazole-resistant fungi , especially TTS-12 also showed in vivo activity against fluconazole-resistant C. albicans .
	manualset3
87677	8	399601	5	NULL	NULL	0	NULL	fluconazole-resistant C. albicans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , steroid saponins TTS-12 and TTS-15 from Tribulus terrestris L. have significant in vitro antifungal activity against fluconazole-resistant fungi , especially TTS-12 also showed in vivo activity against fluconazole-resistant C. albicans .
	manualset3
87679	2	399602	5	NULL	NULL	0	NULL	ADAM17 expression pattern	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the ADAM17 expression pattern and its role in shedding TGF-alpha from cultured human kidney cells suggest a role in the development of fibrosis .
	manualset3
87680	3	399602	5	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the ADAM17 expression pattern and its role in shedding TGF-alpha from cultured human kidney cells suggest a role in the development of fibrosis .
	manualset3
87681	4	399602	5	NULL	NULL	0	NULL	TGF-alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the ADAM17 expression pattern and its role in shedding TGF-alpha from cultured human kidney cells suggest a role in the development of fibrosis .
	manualset3
87682	5	399602	5	NULL	NULL	0	NULL	cultured human kidney cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the ADAM17 expression pattern and its role in shedding TGF-alpha from cultured human kidney cells suggest a role in the development of fibrosis .
	manualset3
87683	6	399602	5	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the ADAM17 expression pattern and its role in shedding TGF-alpha from cultured human kidney cells suggest a role in the development of fibrosis .
	manualset3
87684	7	399602	5	NULL	NULL	0	NULL	development of fibrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the ADAM17 expression pattern and its role in shedding TGF-alpha from cultured human kidney cells suggest a role in the development of fibrosis .
	manualset3
87685	1	399603	5	NULL	NULL	0	NULL	Trabeculectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Trabeculectomy in glaucoma ) .
	manualset3
87686	2	399603	5	NULL	NULL	0	NULL	glaucoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Trabeculectomy in glaucoma ) .
	manualset3
87688	2	399604	5	NULL	NULL	0	NULL	IL-4 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the absence of IL-4 enhanced GC reaction and specific antibody response of Th1-type .
	manualset3
87689	3	399604	5	NULL	NULL	0	NULL	GC reaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the absence of IL-4 enhanced GC reaction and specific antibody response of Th1-type .
	manualset3
87690	4	399604	5	NULL	NULL	0	NULL	specific antibody response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the absence of IL-4 enhanced GC reaction and specific antibody response of Th1-type .
	manualset3
87691	5	399604	5	NULL	NULL	NULL	NULL	Th1-type antibodies	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion , the absence of IL-4 enhanced GC reaction and specific antibody response of Th1-type .
	manualset3
87693	2	399605	5	NULL	NULL	0	NULL	anterolateral thigh flap	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the anterolateral thigh flap is a versatile and dependable flap that can be adapted to any type of defect by modifying the flap design and composition .
	manualset3
87694	3	399605	5	NULL	NULL	0	NULL	versatile and dependable flap	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the anterolateral thigh flap is a versatile and dependable flap that can be adapted to any type of defect by modifying the flap design and composition .
	manualset3
87695	4	399605	5	NULL	NULL	0	NULL	defect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the anterolateral thigh flap is a versatile and dependable flap that can be adapted to any type of defect by modifying the flap design and composition .
	manualset3
87697	2	399606	5	NULL	NULL	0	NULL	expression of YB-1	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the expression of YB-1 in the nucleus is related to carcinogenesis and the development of breast cancer .
	manualset3
87698	3	399606	5	NULL	NULL	0	NULL	nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the expression of YB-1 in the nucleus is related to carcinogenesis and the development of breast cancer .
	manualset3
87699	4	399606	5	NULL	NULL	0	NULL	carcinogenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the expression of YB-1 in the nucleus is related to carcinogenesis and the development of breast cancer .
	manualset3
87700	5	399606	5	NULL	NULL	0	NULL	 development of breast cancer	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the expression of YB-1 in the nucleus is related to carcinogenesis and the development of breast cancer .
	manualset3
87702	1	399607	5	NULL	NULL	NULL	NULL	glass fiber posts	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion , the glass fiber posts proved excellent in flexural strengths and moduli .
	manualset3
87703	1	399608	5	NULL	NULL	0	NULL	new generation of PADPRP inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the new generation of PADPRP inhibitors are at least 50-fold more effective than 3-aminobenzamide as chemopotentiators , and can be used at micromolar rather than millimolar concentrations in intact cells .
	manualset3
87704	2	399608	5	NULL	NULL	0	NULL	3-aminobenzamide	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the new generation of PADPRP inhibitors are at least 50-fold more effective than 3-aminobenzamide as chemopotentiators , and can be used at micromolar rather than millimolar concentrations in intact cells .
	manualset3
87705	3	399608	5	NULL	NULL	0	NULL	chemopotentiators	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the new generation of PADPRP inhibitors are at least 50-fold more effective than 3-aminobenzamide as chemopotentiators , and can be used at micromolar rather than millimolar concentrations in intact cells .
	manualset3
87706	4	399608	5	NULL	NULL	0	NULL	intact cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the new generation of PADPRP inhibitors are at least 50-fold more effective than 3-aminobenzamide as chemopotentiators , and can be used at micromolar rather than millimolar concentrations in intact cells .
	manualset3
87707	1	399609	5	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the present study demonstrates that antagonistic targeting of the histamine H ( 3 ) receptor decreases caloric intake in higher mammalian species .
	manualset3
87708	2	399609	5	NULL	NULL	0	NULL	histamine H ( 3 ) receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the present study demonstrates that antagonistic targeting of the histamine H ( 3 ) receptor decreases caloric intake in higher mammalian species .
	manualset3
87709	3	399609	5	NULL	NULL	0	NULL	caloric intake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the present study demonstrates that antagonistic targeting of the histamine H ( 3 ) receptor decreases caloric intake in higher mammalian species .
	manualset3
87710	4	399609	5	NULL	NULL	0	NULL	higher mammalian species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the present study demonstrates that antagonistic targeting of the histamine H ( 3 ) receptor decreases caloric intake in higher mammalian species .
	manualset3
89568	5	399609	5	NULL	NULL	0	NULL	antagonistic targeting	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the present study demonstrates that antagonistic targeting of the histamine H ( 3 ) receptor decreases caloric intake in higher mammalian species .
	manualset3
87711	1	399610	5	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the present study shows that PTx-sensitivity of receptor-induced ERK1/2 activation could be a consequence of disinhibition of the adenylyl cyclase signaling pathway , which in turn causes inhibition of c-Raf-1 activation rather than indicating involvement of a PTx-sensitive G protein in this signaling pathway .
	manualset3
87712	2	399610	5	NULL	NULL	0	NULL	PTx-sensitivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the present study shows that PTx-sensitivity of receptor-induced ERK1/2 activation could be a consequence of disinhibition of the adenylyl cyclase signaling pathway , which in turn causes inhibition of c-Raf-1 activation rather than indicating involvement of a PTx-sensitive G protein in this signaling pathway .
	manualset3
87713	3	399610	5	NULL	NULL	0	NULL	receptor-induced ERK1/2 activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the present study shows that PTx-sensitivity of receptor-induced ERK1/2 activation could be a consequence of disinhibition of the adenylyl cyclase signaling pathway , which in turn causes inhibition of c-Raf-1 activation rather than indicating involvement of a PTx-sensitive G protein in this signaling pathway .
	manualset3
87714	4	399610	5	NULL	NULL	0	NULL	disinhibition of the adenylyl cyclase signaling pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the present study shows that PTx-sensitivity of receptor-induced ERK1/2 activation could be a consequence of disinhibition of the adenylyl cyclase signaling pathway , which in turn causes inhibition of c-Raf-1 activation rather than indicating involvement of a PTx-sensitive G protein in this signaling pathway .
	manualset3
87715	5	399610	5	NULL	NULL	0	NULL	inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the present study shows that PTx-sensitivity of receptor-induced ERK1/2 activation could be a consequence of disinhibition of the adenylyl cyclase signaling pathway , which in turn causes inhibition of c-Raf-1 activation rather than indicating involvement of a PTx-sensitive G protein in this signaling pathway .
	manualset3
87716	6	399610	5	NULL	NULL	0	NULL	c-Raf-1 activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the present study shows that PTx-sensitivity of receptor-induced ERK1/2 activation could be a consequence of disinhibition of the adenylyl cyclase signaling pathway , which in turn causes inhibition of c-Raf-1 activation rather than indicating involvement of a PTx-sensitive G protein in this signaling pathway .
	manualset3
87717	7	399610	5	NULL	NULL	0	NULL	PTx-sensitive G protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the present study shows that PTx-sensitivity of receptor-induced ERK1/2 activation could be a consequence of disinhibition of the adenylyl cyclase signaling pathway , which in turn causes inhibition of c-Raf-1 activation rather than indicating involvement of a PTx-sensitive G protein in this signaling pathway .
	manualset3
87718	8	399610	5	NULL	NULL	0	NULL	signaling pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the present study shows that PTx-sensitivity of receptor-induced ERK1/2 activation could be a consequence of disinhibition of the adenylyl cyclase signaling pathway , which in turn causes inhibition of c-Raf-1 activation rather than indicating involvement of a PTx-sensitive G protein in this signaling pathway .
	manualset3
87773	1	399611	5	NULL	NULL	0	NULL	polysulfonate resin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the properties of polysulfonate resin , such as particle shape and degree of cross-linking , and the deformation under compaction of fillers affect the physical properties and the drug release of the resinate tablets .
	manualset3
87774	2	399611	5	NULL	NULL	0	NULL	deformation under compaction of fillers	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the properties of polysulfonate resin , such as particle shape and degree of cross-linking , and the deformation under compaction of fillers affect the physical properties and the drug release of the resinate tablets .
	manualset3
87775	3	399611	5	NULL	NULL	0	NULL	drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the properties of polysulfonate resin , such as particle shape and degree of cross-linking , and the deformation under compaction of fillers affect the physical properties and the drug release of the resinate tablets .
	manualset3
87776	4	399611	5	NULL	NULL	0	NULL	resinate tablets	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the properties of polysulfonate resin , such as particle shape and degree of cross-linking , and the deformation under compaction of fillers affect the physical properties and the drug release of the resinate tablets .
	manualset3
87777	1	399612	5	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the study highlighted the rise of non-albicans Candida species in our hospital with differential distribution in paediatric and adult wards and emergence of azole resistance .
	manualset3
87778	2	399612	5	NULL	NULL	0	NULL	non-albicans Candida species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the study highlighted the rise of non-albicans Candida species in our hospital with differential distribution in paediatric and adult wards and emergence of azole resistance .
	manualset3
87779	3	399612	5	NULL	NULL	0	NULL	hospital	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the study highlighted the rise of non-albicans Candida species in our hospital with differential distribution in paediatric and adult wards and emergence of azole resistance .
	manualset3
87780	4	399612	5	NULL	NULL	0	NULL	differential distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the study highlighted the rise of non-albicans Candida species in our hospital with differential distribution in paediatric and adult wards and emergence of azole resistance .
	manualset3
87781	5	399612	5	NULL	NULL	0	NULL	paediatric and adult wards	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the study highlighted the rise of non-albicans Candida species in our hospital with differential distribution in paediatric and adult wards and emergence of azole resistance .
	manualset3
87782	6	399612	5	NULL	NULL	0	NULL	azole resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the study highlighted the rise of non-albicans Candida species in our hospital with differential distribution in paediatric and adult wards and emergence of azole resistance .
	manualset3
87783	1	399613	5	NULL	NULL	0	NULL	Tracheobronchial intracavitary localizations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Tracheobronchial intracavitary localizations of Hodgkin 's disease ) .
	manualset3
87784	2	399613	5	NULL	NULL	0	NULL	Hodgkin 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Tracheobronchial intracavitary localizations of Hodgkin 's disease ) .
	manualset3
87785	1	399614	5	NULL	NULL	0	NULL	MTR profile	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the study of the MTR profile in this myelin lesion model demonstrates in vivo the loss of myelin and the presence of spontaneous remyelination .
	manualset3
87786	2	399614	5	NULL	NULL	NULL	NULL	myelin lesion model	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion , the study of the MTR profile in this myelin lesion model demonstrates in vivo the loss of myelin and the presence of spontaneous remyelination .
	manualset3
87787	3	399614	5	NULL	NULL	0	NULL	loss of myelin	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the study of the MTR profile in this myelin lesion model demonstrates in vivo the loss of myelin and the presence of spontaneous remyelination .
	manualset3
87788	4	399614	5	NULL	NULL	0	NULL	spontaneous remyelination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the study of the MTR profile in this myelin lesion model demonstrates in vivo the loss of myelin and the presence of spontaneous remyelination .
	manualset3
87789	1	399615	5	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the study suggests that GSP are effective in ameliorating the damage to pancreatic tissue in experimental diabetes mellitus .
	manualset3
87790	2	399615	5	NULL	NULL	0	NULL	GSP	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the study suggests that GSP are effective in ameliorating the damage to pancreatic tissue in experimental diabetes mellitus .
	manualset3
87791	3	399615	5	NULL	NULL	0	NULL	pancreatic tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the study suggests that GSP are effective in ameliorating the damage to pancreatic tissue in experimental diabetes mellitus .
	manualset3
87792	4	399615	5	NULL	NULL	0	NULL	experimental diabetes mellitus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the study suggests that GSP are effective in ameliorating the damage to pancreatic tissue in experimental diabetes mellitus .
	manualset3
87793	1	399616	5	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , this study has demonstrated that the long and short cases/orals tested different aspects of student 's skills , and so reinforces the importance of retaining the short and long cases in undergraduate surgical examinations .
	manualset3
87794	2	399616	5	NULL	NULL	NULL	NULL	long and short cases/orals	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion , this study has demonstrated that the long and short cases/orals tested different aspects of student 's skills , and so reinforces the importance of retaining the short and long cases in undergraduate surgical examinations .
	manualset3
87795	3	399616	5	NULL	NULL	NULL	NULL	student 's skills	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion , this study has demonstrated that the long and short cases/orals tested different aspects of student 's skills , and so reinforces the importance of retaining the short and long cases in undergraduate surgical examinations .
	manualset3
87796	4	399616	5	NULL	NULL	NULL	NULL	short and long cases	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion , this study has demonstrated that the long and short cases/orals tested different aspects of student 's skills , and so reinforces the importance of retaining the short and long cases in undergraduate surgical examinations .
	manualset3
87797	5	399616	5	NULL	NULL	NULL	NULL	undergraduate surgical examinations	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion , this study has demonstrated that the long and short cases/orals tested different aspects of student 's skills , and so reinforces the importance of retaining the short and long cases in undergraduate surgical examinations .
	manualset3
87798	1	399617	5	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , this study makes the novel observation that CRP induces IL-8 synthesis and secretion in HAEC via upregulation of NF-kappa B activity .
	manualset3
87799	2	399617	5	NULL	NULL	0	NULL	novel observation	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , this study makes the novel observation that CRP induces IL-8 synthesis and secretion in HAEC via upregulation of NF-kappa B activity .
	manualset3
87800	3	399617	5	NULL	NULL	0	NULL	CRP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , this study makes the novel observation that CRP induces IL-8 synthesis and secretion in HAEC via upregulation of NF-kappa B activity .
	manualset3
87801	4	399617	5	NULL	NULL	0	NULL	IL-8 synthesis and secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , this study makes the novel observation that CRP induces IL-8 synthesis and secretion in HAEC via upregulation of NF-kappa B activity .
	manualset3
87802	5	399617	5	NULL	NULL	0	NULL	HAEC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , this study makes the novel observation that CRP induces IL-8 synthesis and secretion in HAEC via upregulation of NF-kappa B activity .
	manualset3
87803	6	399617	5	NULL	NULL	0	NULL	upregulation of NF-kappa B activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , this study makes the novel observation that CRP induces IL-8 synthesis and secretion in HAEC via upregulation of NF-kappa B activity .
	manualset3
87804	1	399618	5	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , this study shows that developmental increases occur not only in plasma leptin but also in hypothalamic Ob-Rb expression , suggesting that both are likely to influence the timing of puberty onset .
	manualset3
87805	2	399618	5	NULL	NULL	0	NULL	plasma leptin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , this study shows that developmental increases occur not only in plasma leptin but also in hypothalamic Ob-Rb expression , suggesting that both are likely to influence the timing of puberty onset .
	manualset3
87806	3	399618	5	NULL	NULL	0	NULL	hypothalamic Ob-Rb expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , this study shows that developmental increases occur not only in plasma leptin but also in hypothalamic Ob-Rb expression , suggesting that both are likely to influence the timing of puberty onset .
	manualset3
87807	4	399618	5	NULL	NULL	0	NULL	puberty onset	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , this study shows that developmental increases occur not only in plasma leptin but also in hypothalamic Ob-Rb expression , suggesting that both are likely to influence the timing of puberty onset .
	manualset3
89569	5	399618	5	NULL	NULL	0	NULL	developmental increases	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , this study shows that developmental increases occur not only in plasma leptin but also in hypothalamic Ob-Rb expression , suggesting that both are likely to influence the timing of puberty onset .
	manualset3
87808	1	399619	5	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , we did not find any evidence for hepatotoxicity of risperidone rats .
	manualset3
87809	2	399619	5	NULL	NULL	0	NULL	hepatotoxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , we did not find any evidence for hepatotoxicity of risperidone rats .
	manualset3
87810	3	399619	5	NULL	NULL	0	NULL	risperidone rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , we did not find any evidence for hepatotoxicity of risperidone rats .
	manualset3
87811	1	399620	5	NULL	NULL	NULL	NULL	implications	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion , we discuss implications for continued theorizing of the TNSB in light of the experiences of traditionally marginalized populations .
	manualset3
87812	2	399620	5	NULL	NULL	0	NULL	TNSB	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , we discuss implications for continued theorizing of the TNSB in light of the experiences of traditionally marginalized populations .
	manualset3
87813	3	399620	5	NULL	NULL	0	NULL	traditionally marginalized populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , we discuss implications for continued theorizing of the TNSB in light of the experiences of traditionally marginalized populations .
	manualset3
87814	1	399621	5	NULL	NULL	0	NULL	RECQL5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , we propose that RECQL5 stabilises the replication fork allowing replication to overcome the effects of thymidine and complete the cell cycle .
	manualset3
87815	2	399621	5	NULL	NULL	0	NULL	replication fork	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , we propose that RECQL5 stabilises the replication fork allowing replication to overcome the effects of thymidine and complete the cell cycle .
	manualset3
87816	3	399621	5	NULL	NULL	0	NULL	replication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , we propose that RECQL5 stabilises the replication fork allowing replication to overcome the effects of thymidine and complete the cell cycle .
	manualset3
87817	4	399621	5	NULL	NULL	0	NULL	effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , we propose that RECQL5 stabilises the replication fork allowing replication to overcome the effects of thymidine and complete the cell cycle .
	manualset3
87818	5	399621	5	NULL	NULL	0	NULL	thymidine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , we propose that RECQL5 stabilises the replication fork allowing replication to overcome the effects of thymidine and complete the cell cycle .
	manualset3
87819	6	399621	5	NULL	NULL	0	NULL	cell cycle	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , we propose that RECQL5 stabilises the replication fork allowing replication to overcome the effects of thymidine and complete the cell cycle .
	manualset3
87820	1	399622	5	NULL	NULL	0	NULL	non-linear dose-response effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , we suggest non-linear dose-response effect of Halowax 1051 on steroidogenesis and steroidogenic enzymes activity and protein expression .
	manualset3
87821	2	399622	5	NULL	NULL	0	NULL	Halowax 1051	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , we suggest non-linear dose-response effect of Halowax 1051 on steroidogenesis and steroidogenic enzymes activity and protein expression .
	manualset3
87822	3	399622	5	NULL	NULL	0	NULL	steroidogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , we suggest non-linear dose-response effect of Halowax 1051 on steroidogenesis and steroidogenic enzymes activity and protein expression .
	manualset3
87823	4	399622	5	NULL	NULL	0	NULL	steroidogenic enzymes activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , we suggest non-linear dose-response effect of Halowax 1051 on steroidogenesis and steroidogenic enzymes activity and protein expression .
	manualset3
87824	5	399622	5	NULL	NULL	0	NULL	protein expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , we suggest non-linear dose-response effect of Halowax 1051 on steroidogenesis and steroidogenic enzymes activity and protein expression .
	manualset3
87825	1	399623	5	NULL	NULL	0	NULL	Antacids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Antacids and H2 antihistaminics for hyperacidity ) .
	manualset3
87826	2	399623	5	NULL	NULL	0	NULL	H2 antihistaminics	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Antacids and H2 antihistaminics for hyperacidity ) .
	manualset3
87827	3	399623	5	NULL	NULL	0	NULL	hyperacidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Antacids and H2 antihistaminics for hyperacidity ) .
	manualset3
87828	1	399624	5	NULL	NULL	0	NULL	Transient elastography ( FibroScan )	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	( Transient elastography ( FibroScan ) for the non-invasive assessment of liver fibrosis : current status and perspectives ) .
	manualset3
87829	2	399624	5	NULL	NULL	0	NULL	non-invasive assessment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Transient elastography ( FibroScan ) for the non-invasive assessment of liver fibrosis : current status and perspectives ) .
	manualset3
87830	3	399624	5	NULL	NULL	0	NULL	liver fibrosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Transient elastography ( FibroScan ) for the non-invasive assessment of liver fibrosis : current status and perspectives ) .
	manualset3
87831	4	399624	5	NULL	NULL	0	NULL	current status	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Transient elastography ( FibroScan ) for the non-invasive assessment of liver fibrosis : current status and perspectives ) .
	manualset3
87832	5	399624	5	NULL	NULL	0	NULL	perspectives	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Transient elastography ( FibroScan ) for the non-invasive assessment of liver fibrosis : current status and perspectives ) .
	manualset3
87833	1	399625	5	NULL	NULL	0	NULL	creatine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , we were able to demonstrate that the protective potential of creatine was primarily mediated by its impact on cellular energy metabolism and NMDA receptor function , along with reduced glutamate spillover , oxidative stress and subsequent excitotoxicity .
	manualset3
87834	2	399625	5	NULL	NULL	0	NULL	impact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , we were able to demonstrate that the protective potential of creatine was primarily mediated by its impact on cellular energy metabolism and NMDA receptor function , along with reduced glutamate spillover , oxidative stress and subsequent excitotoxicity .
	manualset3
87835	3	399625	5	NULL	NULL	0	NULL	cellular energy metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , we were able to demonstrate that the protective potential of creatine was primarily mediated by its impact on cellular energy metabolism and NMDA receptor function , along with reduced glutamate spillover , oxidative stress and subsequent excitotoxicity .
	manualset3
87836	4	399625	5	NULL	NULL	0	NULL	NMDA receptor function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , we were able to demonstrate that the protective potential of creatine was primarily mediated by its impact on cellular energy metabolism and NMDA receptor function , along with reduced glutamate spillover , oxidative stress and subsequent excitotoxicity .
	manualset3
87837	5	399625	5	NULL	NULL	0	NULL	reduced glutamate spillover	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , we were able to demonstrate that the protective potential of creatine was primarily mediated by its impact on cellular energy metabolism and NMDA receptor function , along with reduced glutamate spillover , oxidative stress and subsequent excitotoxicity .
	manualset3
87839	6	399625	5	NULL	NULL	0	NULL	oxidative stress	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , we were able to demonstrate that the protective potential of creatine was primarily mediated by its impact on cellular energy metabolism and NMDA receptor function , along with reduced glutamate spillover , oxidative stress and subsequent excitotoxicity .
	manualset3
87840	7	399625	5	NULL	NULL	0	NULL	subsequent excitotoxicity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , we were able to demonstrate that the protective potential of creatine was primarily mediated by its impact on cellular energy metabolism and NMDA receptor function , along with reduced glutamate spillover , oxidative stress and subsequent excitotoxicity .
	manualset3
87841	1	399626	5	NULL	NULL	0	NULL	long periods of time ( 9.5 months to 2 years )	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , when given for long periods of time ( 9.5 months to 2 years ) , LTG was well tolerated in doses up to 400 mg/day and mean trough levels of 3.0 + / - 0.6 microgram/ml ; LTG has a favorable pharmacokinetic profile and appears to exhibit first-order linear kinetics during long-term chronic dosing ; LTG shows preliminary evidence of efficacy during long-term administration ; and to date , our patients represent the longest reported experience of continuous and closely monitored LTG therapy in the literature .
	manualset3
87842	2	399626	5	NULL	NULL	0	NULL	LTG	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , when given for long periods of time ( 9.5 months to 2 years ) , LTG was well tolerated in doses up to 400 mg/day and mean trough levels of 3.0 + / - 0.6 microgram/ml ; LTG has a favorable pharmacokinetic profile and appears to exhibit first-order linear kinetics during long-term chronic dosing ; LTG shows preliminary evidence of efficacy during long-term administration ; and to date , our patients represent the longest reported experience of continuous and closely monitored LTG therapy in the literature .
	manualset3
87843	3	399626	5	NULL	NULL	0	NULL	doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , when given for long periods of time ( 9.5 months to 2 years ) , LTG was well tolerated in doses up to 400 mg/day and mean trough levels of 3.0 + / - 0.6 microgram/ml ; LTG has a favorable pharmacokinetic profile and appears to exhibit first-order linear kinetics during long-term chronic dosing ; LTG shows preliminary evidence of efficacy during long-term administration ; and to date , our patients represent the longest reported experience of continuous and closely monitored LTG therapy in the literature .
	manualset3
87844	4	399626	5	NULL	NULL	0	NULL	400 mg/day	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , when given for long periods of time ( 9.5 months to 2 years ) , LTG was well tolerated in doses up to 400 mg/day and mean trough levels of 3.0 + / - 0.6 microgram/ml ; LTG has a favorable pharmacokinetic profile and appears to exhibit first-order linear kinetics during long-term chronic dosing ; LTG shows preliminary evidence of efficacy during long-term administration ; and to date , our patients represent the longest reported experience of continuous and closely monitored LTG therapy in the literature .
	manualset3
87845	5	399626	5	NULL	NULL	0	NULL	mean trough levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , when given for long periods of time ( 9.5 months to 2 years ) , LTG was well tolerated in doses up to 400 mg/day and mean trough levels of 3.0 + / - 0.6 microgram/ml ; LTG has a favorable pharmacokinetic profile and appears to exhibit first-order linear kinetics during long-term chronic dosing ; LTG shows preliminary evidence of efficacy during long-term administration ; and to date , our patients represent the longest reported experience of continuous and closely monitored LTG therapy in the literature .
	manualset3
87846	6	399626	5	NULL	NULL	0	NULL	3.0 + / - 0.6 microgram/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , when given for long periods of time ( 9.5 months to 2 years ) , LTG was well tolerated in doses up to 400 mg/day and mean trough levels of 3.0 + / - 0.6 microgram/ml ; LTG has a favorable pharmacokinetic profile and appears to exhibit first-order linear kinetics during long-term chronic dosing ; LTG shows preliminary evidence of efficacy during long-term administration ; and to date , our patients represent the longest reported experience of continuous and closely monitored LTG therapy in the literature .
	manualset3
87847	7	399626	5	NULL	NULL	0	NULL	LTG	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , when given for long periods of time ( 9.5 months to 2 years ) , LTG was well tolerated in doses up to 400 mg/day and mean trough levels of 3.0 + / - 0.6 microgram/ml ; LTG has a favorable pharmacokinetic profile and appears to exhibit first-order linear kinetics during long-term chronic dosing ; LTG shows preliminary evidence of efficacy during long-term administration ; and to date , our patients represent the longest reported experience of continuous and closely monitored LTG therapy in the literature .
	manualset3
87848	8	399626	5	NULL	NULL	NULL	NULL	favorable pharmacokinetic profile	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion , when given for long periods of time ( 9.5 months to 2 years ) , LTG was well tolerated in doses up to 400 mg/day and mean trough levels of 3.0 + / - 0.6 microgram/ml ; LTG has a favorable pharmacokinetic profile and appears to exhibit first-order linear kinetics during long-term chronic dosing ; LTG shows preliminary evidence of efficacy during long-term administration ; and to date , our patients represent the longest reported experience of continuous and closely monitored LTG therapy in the literature .
	manualset3
87849	9	399626	5	NULL	NULL	0	NULL	first-order linear kinetics	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , when given for long periods of time ( 9.5 months to 2 years ) , LTG was well tolerated in doses up to 400 mg/day and mean trough levels of 3.0 + / - 0.6 microgram/ml ; LTG has a favorable pharmacokinetic profile and appears to exhibit first-order linear kinetics during long-term chronic dosing ; LTG shows preliminary evidence of efficacy during long-term administration ; and to date , our patients represent the longest reported experience of continuous and closely monitored LTG therapy in the literature .
	manualset3
87850	10	399626	5	NULL	NULL	0	NULL	LTG	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , when given for long periods of time ( 9.5 months to 2 years ) , LTG was well tolerated in doses up to 400 mg/day and mean trough levels of 3.0 + / - 0.6 microgram/ml ; LTG has a favorable pharmacokinetic profile and appears to exhibit first-order linear kinetics during long-term chronic dosing ; LTG shows preliminary evidence of efficacy during long-term administration ; and to date , our patients represent the longest reported experience of continuous and closely monitored LTG therapy in the literature .
	manualset3
87851	11	399626	5	NULL	NULL	NULL	NULL	efficacy	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion , when given for long periods of time ( 9.5 months to 2 years ) , LTG was well tolerated in doses up to 400 mg/day and mean trough levels of 3.0 + / - 0.6 microgram/ml ; LTG has a favorable pharmacokinetic profile and appears to exhibit first-order linear kinetics during long-term chronic dosing ; LTG shows preliminary evidence of efficacy during long-term administration ; and to date , our patients represent the longest reported experience of continuous and closely monitored LTG therapy in the literature .
	manualset3
87852	12	399626	5	NULL	NULL	0	NULL	long-term administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , when given for long periods of time ( 9.5 months to 2 years ) , LTG was well tolerated in doses up to 400 mg/day and mean trough levels of 3.0 + / - 0.6 microgram/ml ; LTG has a favorable pharmacokinetic profile and appears to exhibit first-order linear kinetics during long-term chronic dosing ; LTG shows preliminary evidence of efficacy during long-term administration ; and to date , our patients represent the longest reported experience of continuous and closely monitored LTG therapy in the literature .
	manualset3
87853	13	399626	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , when given for long periods of time ( 9.5 months to 2 years ) , LTG was well tolerated in doses up to 400 mg/day and mean trough levels of 3.0 + / - 0.6 microgram/ml ; LTG has a favorable pharmacokinetic profile and appears to exhibit first-order linear kinetics during long-term chronic dosing ; LTG shows preliminary evidence of efficacy during long-term administration ; and to date , our patients represent the longest reported experience of continuous and closely monitored LTG therapy in the literature .
	manualset3
87854	14	399626	5	NULL	NULL	0	NULL	experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , when given for long periods of time ( 9.5 months to 2 years ) , LTG was well tolerated in doses up to 400 mg/day and mean trough levels of 3.0 + / - 0.6 microgram/ml ; LTG has a favorable pharmacokinetic profile and appears to exhibit first-order linear kinetics during long-term chronic dosing ; LTG shows preliminary evidence of efficacy during long-term administration ; and to date , our patients represent the longest reported experience of continuous and closely monitored LTG therapy in the literature .
	manualset3
87855	15	399626	5	NULL	NULL	0	NULL	LTG therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , when given for long periods of time ( 9.5 months to 2 years ) , LTG was well tolerated in doses up to 400 mg/day and mean trough levels of 3.0 + / - 0.6 microgram/ml ; LTG has a favorable pharmacokinetic profile and appears to exhibit first-order linear kinetics during long-term chronic dosing ; LTG shows preliminary evidence of efficacy during long-term administration ; and to date , our patients represent the longest reported experience of continuous and closely monitored LTG therapy in the literature .
	manualset3
87856	16	399626	5	NULL	NULL	0	NULL	literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , when given for long periods of time ( 9.5 months to 2 years ) , LTG was well tolerated in doses up to 400 mg/day and mean trough levels of 3.0 + / - 0.6 microgram/ml ; LTG has a favorable pharmacokinetic profile and appears to exhibit first-order linear kinetics during long-term chronic dosing ; LTG shows preliminary evidence of efficacy during long-term administration ; and to date , our patients represent the longest reported experience of continuous and closely monitored LTG therapy in the literature .
	manualset3
88115	17	399626	5	NULL	NULL	0	NULL	long-term chronic dosing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , when given for long periods of time ( 9.5 months to 2 years ) , LTG was well tolerated in doses up to 400 mg/day and mean trough levels of 3.0 + / - 0.6 microgram/ml ; LTG has a favorable pharmacokinetic profile and appears to exhibit first-order linear kinetics during long-term chronic dosing ; LTG shows preliminary evidence of efficacy during long-term administration ; and to date , our patients represent the longest reported experience of continuous and closely monitored LTG therapy in the literature .
	manualset3
87857	1	399627	5	NULL	NULL	0	NULL	VE	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , while VE can not replace endoscopy of the tracheobronchial tree or the oesophagus , it is an accurate and non-invasive method for identifying endoluminal tumors , grading stenoses and visualizing the tracheobronchial tree beyond stenoses in a small number of patients who are not amenable to endoscopy .
	manualset3
87858	2	399627	5	NULL	NULL	0	NULL	endoscopy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , while VE can not replace endoscopy of the tracheobronchial tree or the oesophagus , it is an accurate and non-invasive method for identifying endoluminal tumors , grading stenoses and visualizing the tracheobronchial tree beyond stenoses in a small number of patients who are not amenable to endoscopy .
	manualset3
87859	3	399627	5	NULL	NULL	0	NULL	tracheobronchial tree	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , while VE can not replace endoscopy of the tracheobronchial tree or the oesophagus , it is an accurate and non-invasive method for identifying endoluminal tumors , grading stenoses and visualizing the tracheobronchial tree beyond stenoses in a small number of patients who are not amenable to endoscopy .
	manualset3
87860	4	399627	5	NULL	NULL	0	NULL	oesophagus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , while VE can not replace endoscopy of the tracheobronchial tree or the oesophagus , it is an accurate and non-invasive method for identifying endoluminal tumors , grading stenoses and visualizing the tracheobronchial tree beyond stenoses in a small number of patients who are not amenable to endoscopy .
	manualset3
87861	5	399627	5	NULL	NULL	0	NULL	endoluminal tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , while VE can not replace endoscopy of the tracheobronchial tree or the oesophagus , it is an accurate and non-invasive method for identifying endoluminal tumors , grading stenoses and visualizing the tracheobronchial tree beyond stenoses in a small number of patients who are not amenable to endoscopy .
	manualset3
87862	6	399627	5	NULL	NULL	0	NULL	grading stenoses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , while VE can not replace endoscopy of the tracheobronchial tree or the oesophagus , it is an accurate and non-invasive method for identifying endoluminal tumors , grading stenoses and visualizing the tracheobronchial tree beyond stenoses in a small number of patients who are not amenable to endoscopy .
	manualset3
87863	7	399627	5	NULL	NULL	0	NULL	tracheobronchial tree	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , while VE can not replace endoscopy of the tracheobronchial tree or the oesophagus , it is an accurate and non-invasive method for identifying endoluminal tumors , grading stenoses and visualizing the tracheobronchial tree beyond stenoses in a small number of patients who are not amenable to endoscopy .
	manualset3
87864	8	399627	5	NULL	NULL	0	NULL	stenoses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , while VE can not replace endoscopy of the tracheobronchial tree or the oesophagus , it is an accurate and non-invasive method for identifying endoluminal tumors , grading stenoses and visualizing the tracheobronchial tree beyond stenoses in a small number of patients who are not amenable to endoscopy .
	manualset3
87865	9	399627	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , while VE can not replace endoscopy of the tracheobronchial tree or the oesophagus , it is an accurate and non-invasive method for identifying endoluminal tumors , grading stenoses and visualizing the tracheobronchial tree beyond stenoses in a small number of patients who are not amenable to endoscopy .
	manualset3
87866	10	399627	5	NULL	NULL	0	NULL	endoscopy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , while VE can not replace endoscopy of the tracheobronchial tree or the oesophagus , it is an accurate and non-invasive method for identifying endoluminal tumors , grading stenoses and visualizing the tracheobronchial tree beyond stenoses in a small number of patients who are not amenable to endoscopy .
	manualset3
87867	1	399628	5	NULL	NULL	0	NULL	xenogeneic transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , xenogeneic transplantation of human PBSCs into NOD/SCID mice provides an excellent in vivo model to study human megakaryocytopoiesis and platelet production .
	manualset3
87868	2	399628	5	NULL	NULL	0	NULL	human PBSCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , xenogeneic transplantation of human PBSCs into NOD/SCID mice provides an excellent in vivo model to study human megakaryocytopoiesis and platelet production .
	manualset3
87869	3	399628	5	NULL	NULL	0	NULL	NOD/SCID mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , xenogeneic transplantation of human PBSCs into NOD/SCID mice provides an excellent in vivo model to study human megakaryocytopoiesis and platelet production .
	manualset3
87870	4	399628	5	NULL	NULL	NULL	NULL	 in vivo model	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion , xenogeneic transplantation of human PBSCs into NOD/SCID mice provides an excellent in vivo model to study human megakaryocytopoiesis and platelet production .
	manualset3
87871	5	399628	5	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , xenogeneic transplantation of human PBSCs into NOD/SCID mice provides an excellent in vivo model to study human megakaryocytopoiesis and platelet production .
	manualset3
87872	6	399628	5	NULL	NULL	0	NULL	human megakaryocytopoiesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , xenogeneic transplantation of human PBSCs into NOD/SCID mice provides an excellent in vivo model to study human megakaryocytopoiesis and platelet production .
	manualset3
87873	7	399628	5	NULL	NULL	0	NULL	platelet production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , xenogeneic transplantation of human PBSCs into NOD/SCID mice provides an excellent in vivo model to study human megakaryocytopoiesis and platelet production .
	manualset3
87874	1	399629	5	NULL	NULL	0	NULL	zinc	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , zinc activates KATP by binding itself to extracellular His-326 and His-332 of the SUR1 subunit .
	manualset3
87875	2	399629	5	NULL	NULL	0	NULL	KATP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , zinc activates KATP by binding itself to extracellular His-326 and His-332 of the SUR1 subunit .
	manualset3
87876	3	399629	5	NULL	NULL	0	NULL	extracellular His-326	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , zinc activates KATP by binding itself to extracellular His-326 and His-332 of the SUR1 subunit .
	manualset3
87877	4	399629	5	NULL	NULL	0	NULL	His-332	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , zinc activates KATP by binding itself to extracellular His-326 and His-332 of the SUR1 subunit .
	manualset3
87878	5	399629	5	NULL	NULL	0	NULL	SUR1 subunit	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , zinc activates KATP by binding itself to extracellular His-326 and His-332 of the SUR1 subunit .
	manualset3
87879	1	399630	5	NULL	NULL	0	NULL	Ca ( 2 + )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In controls , Ca ( 2 + ) load required for mPTP opening averaged 11 + / - 4 microM mg ( -1 ) mitochondrial protein versus 116 + / - 6 in shams ( P & lt ; 0.0001 ) .
	manualset3
87880	2	399630	5	NULL	NULL	NULL	NULL	mPTP opening	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In controls , Ca ( 2 + ) load required for mPTP opening averaged 11 + / - 4 microM mg ( -1 ) mitochondrial protein versus 116 + / - 6 in shams ( P & lt ; 0.0001 ) .
	manualset3
87881	3	399630	5	NULL	NULL	0	NULL	11 + / - 4 microM mg ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In controls , Ca ( 2 + ) load required for mPTP opening averaged 11 + / - 4 microM mg ( -1 ) mitochondrial protein versus 116 + / - 6 in shams ( P & lt ; 0.0001 ) .
	manualset3
87882	4	399630	5	NULL	NULL	0	NULL	mitochondrial protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In controls , Ca ( 2 + ) load required for mPTP opening averaged 11 + / - 4 microM mg ( -1 ) mitochondrial protein versus 116 + / - 6 in shams ( P & lt ; 0.0001 ) .
	manualset3
87883	5	399630	5	NULL	NULL	0	NULL	116 + / - 6	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In controls , Ca ( 2 + ) load required for mPTP opening averaged 11 + / - 4 microM mg ( -1 ) mitochondrial protein versus 116 + / - 6 in shams ( P & lt ; 0.0001 ) .
	manualset3
87884	6	399630	5	NULL	NULL	0	NULL	shams	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In controls , Ca ( 2 + ) load required for mPTP opening averaged 11 + / - 4 microM mg ( -1 ) mitochondrial protein versus 116 + / - 6 in shams ( P & lt ; 0.0001 ) .
	manualset3
87885	7	399630	5	NULL	NULL	0	NULL	P & lt ; 0.0001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In controls , Ca ( 2 + ) load required for mPTP opening averaged 11 + / - 4 microM mg ( -1 ) mitochondrial protein versus 116 + / - 6 in shams ( P & lt ; 0.0001 ) .
	manualset3
88116	1	399631	5	NULL	NULL	0	NULL	eukaryotes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In eukaryotes , manganese superoxide dismutase is a nuclear-encoded protein that scavenges superoxide radicals in the mitochondrial matrix .
	manualset3
88117	2	399631	5	NULL	NULL	0	NULL	manganese superoxide dismutase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In eukaryotes , manganese superoxide dismutase is a nuclear-encoded protein that scavenges superoxide radicals in the mitochondrial matrix .
	manualset3
88118	3	399631	5	NULL	NULL	0	NULL	nuclear-encoded protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In eukaryotes , manganese superoxide dismutase is a nuclear-encoded protein that scavenges superoxide radicals in the mitochondrial matrix .
	manualset3
88119	4	399631	5	NULL	NULL	0	NULL	superoxide radicals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In eukaryotes , manganese superoxide dismutase is a nuclear-encoded protein that scavenges superoxide radicals in the mitochondrial matrix .
	manualset3
88120	5	399631	5	NULL	NULL	0	NULL	mitochondrial matrix	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In eukaryotes , manganese superoxide dismutase is a nuclear-encoded protein that scavenges superoxide radicals in the mitochondrial matrix .
	manualset3
88121	1	399632	5	NULL	NULL	NULL	NULL	excised , inside-out patches	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In excised , inside-out patches , it was demonstrated that ATP currents were mediated by ATP-conductive channels , which were also activated by protein kinase A and blocked by the Cl - channel blocker diphenylamine-2-carboxylate under excised , inside-out conditions .
	manualset3
88122	2	399632	5	NULL	NULL	0	NULL	ATP currents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In excised , inside-out patches , it was demonstrated that ATP currents were mediated by ATP-conductive channels , which were also activated by protein kinase A and blocked by the Cl - channel blocker diphenylamine-2-carboxylate under excised , inside-out conditions .
	manualset3
88123	3	399632	5	NULL	NULL	0	NULL	ATP-conductive channels	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In excised , inside-out patches , it was demonstrated that ATP currents were mediated by ATP-conductive channels , which were also activated by protein kinase A and blocked by the Cl - channel blocker diphenylamine-2-carboxylate under excised , inside-out conditions .
	manualset3
88124	4	399632	5	NULL	NULL	0	NULL	protein kinase A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In excised , inside-out patches , it was demonstrated that ATP currents were mediated by ATP-conductive channels , which were also activated by protein kinase A and blocked by the Cl - channel blocker diphenylamine-2-carboxylate under excised , inside-out conditions .
	manualset3
88125	5	399632	5	NULL	NULL	0	NULL	Cl - channel blocker diphenylamine-2-carboxylate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In excised , inside-out patches , it was demonstrated that ATP currents were mediated by ATP-conductive channels , which were also activated by protein kinase A and blocked by the Cl - channel blocker diphenylamine-2-carboxylate under excised , inside-out conditions .
	manualset3
88126	6	399632	5	NULL	NULL	NULL	NULL	excised , inside-out conditions	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In excised , inside-out patches , it was demonstrated that ATP currents were mediated by ATP-conductive channels , which were also activated by protein kinase A and blocked by the Cl - channel blocker diphenylamine-2-carboxylate under excised , inside-out conditions .
	manualset3
88127	1	399633	5	NULL	NULL	0	NULL	experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In experiments in vitro against Mycobacterium tuberculosis , these compounds displayed minimum inhibitory concentration ( MIC ) values between several fold and several hundred fold greater than that of INH itself , on a molar basis , with some of the more active compounds having higher calculated values of log P. Among these derivatives , compound 1b , closely homologous to the INH metabolite 1a , N2-acetylisoniazid , provided unexpected protection in tuberculosis-infected mice .
	manualset3
88128	2	399633	5	NULL	NULL	NULL	NULL	Mycobacterium tuberculosis	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In experiments in vitro against Mycobacterium tuberculosis , these compounds displayed minimum inhibitory concentration ( MIC ) values between several fold and several hundred fold greater than that of INH itself , on a molar basis , with some of the more active compounds having higher calculated values of log P. Among these derivatives , compound 1b , closely homologous to the INH metabolite 1a , N2-acetylisoniazid , provided unexpected protection in tuberculosis-infected mice .
	manualset3
88129	3	399633	5	NULL	NULL	0	NULL	compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In experiments in vitro against Mycobacterium tuberculosis , these compounds displayed minimum inhibitory concentration ( MIC ) values between several fold and several hundred fold greater than that of INH itself , on a molar basis , with some of the more active compounds having higher calculated values of log P. Among these derivatives , compound 1b , closely homologous to the INH metabolite 1a , N2-acetylisoniazid , provided unexpected protection in tuberculosis-infected mice .
	manualset3
88187	4	399633	5	NULL	NULL	0	NULL	minimum inhibitory concentration ( MIC ) values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In experiments in vitro against Mycobacterium tuberculosis , these compounds displayed minimum inhibitory concentration ( MIC ) values between several fold and several hundred fold greater than that of INH itself , on a molar basis , with some of the more active compounds having higher calculated values of log P. Among these derivatives , compound 1b , closely homologous to the INH metabolite 1a , N2-acetylisoniazid , provided unexpected protection in tuberculosis-infected mice .
	manualset3
88188	5	399633	5	NULL	NULL	0	NULL	INH	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In experiments in vitro against Mycobacterium tuberculosis , these compounds displayed minimum inhibitory concentration ( MIC ) values between several fold and several hundred fold greater than that of INH itself , on a molar basis , with some of the more active compounds having higher calculated values of log P. Among these derivatives , compound 1b , closely homologous to the INH metabolite 1a , N2-acetylisoniazid , provided unexpected protection in tuberculosis-infected mice .
	manualset3
88189	6	399633	5	NULL	NULL	0	NULL	molar basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In experiments in vitro against Mycobacterium tuberculosis , these compounds displayed minimum inhibitory concentration ( MIC ) values between several fold and several hundred fold greater than that of INH itself , on a molar basis , with some of the more active compounds having higher calculated values of log P. Among these derivatives , compound 1b , closely homologous to the INH metabolite 1a , N2-acetylisoniazid , provided unexpected protection in tuberculosis-infected mice .
	manualset3
88190	7	399633	5	NULL	NULL	0	NULL	active compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In experiments in vitro against Mycobacterium tuberculosis , these compounds displayed minimum inhibitory concentration ( MIC ) values between several fold and several hundred fold greater than that of INH itself , on a molar basis , with some of the more active compounds having higher calculated values of log P. Among these derivatives , compound 1b , closely homologous to the INH metabolite 1a , N2-acetylisoniazid , provided unexpected protection in tuberculosis-infected mice .
	manualset3
88191	8	399633	5	NULL	NULL	0	NULL	log P	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In experiments in vitro against Mycobacterium tuberculosis , these compounds displayed minimum inhibitory concentration ( MIC ) values between several fold and several hundred fold greater than that of INH itself , on a molar basis , with some of the more active compounds having higher calculated values of log P. Among these derivatives , compound 1b , closely homologous to the INH metabolite 1a , N2-acetylisoniazid , provided unexpected protection in tuberculosis-infected mice .
	manualset3
88192	9	399633	5	NULL	NULL	0	NULL	derivatives	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In experiments in vitro against Mycobacterium tuberculosis , these compounds displayed minimum inhibitory concentration ( MIC ) values between several fold and several hundred fold greater than that of INH itself , on a molar basis , with some of the more active compounds having higher calculated values of log P. Among these derivatives , compound 1b , closely homologous to the INH metabolite 1a , N2-acetylisoniazid , provided unexpected protection in tuberculosis-infected mice .
	manualset3
88193	10	399633	5	NULL	NULL	0	NULL	compound 1b	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In experiments in vitro against Mycobacterium tuberculosis , these compounds displayed minimum inhibitory concentration ( MIC ) values between several fold and several hundred fold greater than that of INH itself , on a molar basis , with some of the more active compounds having higher calculated values of log P. Among these derivatives , compound 1b , closely homologous to the INH metabolite 1a , N2-acetylisoniazid , provided unexpected protection in tuberculosis-infected mice .
	manualset3
88194	11	399633	5	NULL	NULL	0	NULL	INH metabolite 1a	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In experiments in vitro against Mycobacterium tuberculosis , these compounds displayed minimum inhibitory concentration ( MIC ) values between several fold and several hundred fold greater than that of INH itself , on a molar basis , with some of the more active compounds having higher calculated values of log P. Among these derivatives , compound 1b , closely homologous to the INH metabolite 1a , N2-acetylisoniazid , provided unexpected protection in tuberculosis-infected mice .
	manualset3
88195	12	399633	5	NULL	NULL	0	NULL	N2-acetylisoniazid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In experiments in vitro against Mycobacterium tuberculosis , these compounds displayed minimum inhibitory concentration ( MIC ) values between several fold and several hundred fold greater than that of INH itself , on a molar basis , with some of the more active compounds having higher calculated values of log P. Among these derivatives , compound 1b , closely homologous to the INH metabolite 1a , N2-acetylisoniazid , provided unexpected protection in tuberculosis-infected mice .
	manualset3
88196	13	399633	5	NULL	NULL	0	NULL	protection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In experiments in vitro against Mycobacterium tuberculosis , these compounds displayed minimum inhibitory concentration ( MIC ) values between several fold and several hundred fold greater than that of INH itself , on a molar basis , with some of the more active compounds having higher calculated values of log P. Among these derivatives , compound 1b , closely homologous to the INH metabolite 1a , N2-acetylisoniazid , provided unexpected protection in tuberculosis-infected mice .
	manualset3
88197	14	399633	5	NULL	NULL	0	NULL	tuberculosis-infected mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In experiments in vitro against Mycobacterium tuberculosis , these compounds displayed minimum inhibitory concentration ( MIC ) values between several fold and several hundred fold greater than that of INH itself , on a molar basis , with some of the more active compounds having higher calculated values of log P. Among these derivatives , compound 1b , closely homologous to the INH metabolite 1a , N2-acetylisoniazid , provided unexpected protection in tuberculosis-infected mice .
	manualset3
88198	1	399634	5	NULL	NULL	0	NULL	45 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In fact , it has been estimated that approximately 45 % of epigenetic researchers today identify cancer/oncology as their main area of focus vis -- vis their epigenetic research efforts .
	manualset3
88199	2	399634	5	NULL	NULL	0	NULL	epigenetic researchers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In fact , it has been estimated that approximately 45 % of epigenetic researchers today identify cancer/oncology as their main area of focus vis -- vis their epigenetic research efforts .
	manualset3
88200	3	399634	5	NULL	NULL	0	NULL	cancer/oncology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In fact , it has been estimated that approximately 45 % of epigenetic researchers today identify cancer/oncology as their main area of focus vis -- vis their epigenetic research efforts .
	manualset3
88201	4	399634	5	NULL	NULL	0	NULL	main area of focus	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In fact , it has been estimated that approximately 45 % of epigenetic researchers today identify cancer/oncology as their main area of focus vis -- vis their epigenetic research efforts .
	manualset3
88202	5	399634	5	NULL	NULL	0	NULL	epigenetic research efforts	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In fact , it has been estimated that approximately 45 % of epigenetic researchers today identify cancer/oncology as their main area of focus vis -- vis their epigenetic research efforts .
	manualset3
88203	1	399635	5	NULL	NULL	0	NULL	spatial-temporal values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In fact , these spatial-temporal values were stable during the time spent stroking and were higher or lower during the start , the turns ( in and out ) , and the finish .
	manualset3
88204	2	399635	5	NULL	NULL	0	NULL	time spent stroking	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In fact , these spatial-temporal values were stable during the time spent stroking and were higher or lower during the start , the turns ( in and out ) , and the finish .
	manualset3
88205	3	399635	5	NULL	NULL	0	NULL	start	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In fact , these spatial-temporal values were stable during the time spent stroking and were higher or lower during the start , the turns ( in and out ) , and the finish .
	manualset3
88206	4	399635	5	NULL	NULL	0	NULL	turns ( in and out )	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In fact , these spatial-temporal values were stable during the time spent stroking and were higher or lower during the start , the turns ( in and out ) , and the finish .
	manualset3
88207	5	399635	5	NULL	NULL	0	NULL	finish	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In fact , these spatial-temporal values were stable during the time spent stroking and were higher or lower during the start , the turns ( in and out ) , and the finish .
	manualset3
88208	1	399636	5	NULL	NULL	0	NULL	females	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In females , the weight-related development of menarche leads to earlier menarche in obese girls than in normal weight girls .
	manualset3
88209	2	399636	5	NULL	NULL	0	NULL	weight-related development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In females , the weight-related development of menarche leads to earlier menarche in obese girls than in normal weight girls .
	manualset3
88210	3	399636	5	NULL	NULL	0	NULL	menarche	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In females , the weight-related development of menarche leads to earlier menarche in obese girls than in normal weight girls .
	manualset3
88211	4	399636	5	NULL	NULL	0	NULL	earlier menarche	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In females , the weight-related development of menarche leads to earlier menarche in obese girls than in normal weight girls .
	manualset3
88212	5	399636	5	NULL	NULL	0	NULL	obese girls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In females , the weight-related development of menarche leads to earlier menarche in obese girls than in normal weight girls .
	manualset3
88213	6	399636	5	NULL	NULL	0	NULL	normal weight girls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In females , the weight-related development of menarche leads to earlier menarche in obese girls than in normal weight girls .
	manualset3
88214	1	399637	5	NULL	NULL	NULL	NULL	future	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In future , the choice of the ideal volume replacement regimen should not only be focused on its volume restoring properties , but additional effects ( e.g. on organ perfusion on , tissue oxygenation , inflammation , endothelial activation , capillary leakage ) should also be taken into account when treating hypovolemia in the critically ill .
	manualset3
88349	2	399637	5	NULL	NULL	NULL	NULL	 ideal volume replacement regimen	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In future , the choice of the ideal volume replacement regimen should not only be focused on its volume restoring properties , but additional effects ( e.g. on organ perfusion on , tissue oxygenation , inflammation , endothelial activation , capillary leakage ) should also be taken into account when treating hypovolemia in the critically ill .
	manualset3
88353	3	399637	5	NULL	NULL	0	NULL	additional effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In future , the choice of the ideal volume replacement regimen should not only be focused on its volume restoring properties , but additional effects ( e.g. on organ perfusion on , tissue oxygenation , inflammation , endothelial activation , capillary leakage ) should also be taken into account when treating hypovolemia in the critically ill .
	manualset3
88354	4	399637	5	NULL	NULL	0	NULL	organ perfusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In future , the choice of the ideal volume replacement regimen should not only be focused on its volume restoring properties , but additional effects ( e.g. on organ perfusion on , tissue oxygenation , inflammation , endothelial activation , capillary leakage ) should also be taken into account when treating hypovolemia in the critically ill .
	manualset3
88355	5	399637	5	NULL	NULL	NULL	NULL	tissue oxygenation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In future , the choice of the ideal volume replacement regimen should not only be focused on its volume restoring properties , but additional effects ( e.g. on organ perfusion on , tissue oxygenation , inflammation , endothelial activation , capillary leakage ) should also be taken into account when treating hypovolemia in the critically ill .
	manualset3
88356	6	399637	5	NULL	NULL	0	NULL	inflammation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In future , the choice of the ideal volume replacement regimen should not only be focused on its volume restoring properties , but additional effects ( e.g. on organ perfusion on , tissue oxygenation , inflammation , endothelial activation , capillary leakage ) should also be taken into account when treating hypovolemia in the critically ill .
	manualset3
88357	7	399637	5	NULL	NULL	0	NULL	endothelial activation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In future , the choice of the ideal volume replacement regimen should not only be focused on its volume restoring properties , but additional effects ( e.g. on organ perfusion on , tissue oxygenation , inflammation , endothelial activation , capillary leakage ) should also be taken into account when treating hypovolemia in the critically ill .
	manualset3
88358	8	399637	5	NULL	NULL	0	NULL	capillary leakage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In future , the choice of the ideal volume replacement regimen should not only be focused on its volume restoring properties , but additional effects ( e.g. on organ perfusion on , tissue oxygenation , inflammation , endothelial activation , capillary leakage ) should also be taken into account when treating hypovolemia in the critically ill .
	manualset3
88359	9	399637	5	NULL	NULL	0	NULL	hypovolemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In future , the choice of the ideal volume replacement regimen should not only be focused on its volume restoring properties , but additional effects ( e.g. on organ perfusion on , tissue oxygenation , inflammation , endothelial activation , capillary leakage ) should also be taken into account when treating hypovolemia in the critically ill .
	manualset3
88360	10	399637	5	NULL	NULL	0	NULL	critically ill	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In future , the choice of the ideal volume replacement regimen should not only be focused on its volume restoring properties , but additional effects ( e.g. on organ perfusion on , tissue oxygenation , inflammation , endothelial activation , capillary leakage ) should also be taken into account when treating hypovolemia in the critically ill .
	manualset3
88361	11	399637	5	NULL	NULL	0	NULL	choice	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In future , the choice of the ideal volume replacement regimen should not only be focused on its volume restoring properties , but additional effects ( e.g. on organ perfusion on , tissue oxygenation , inflammation , endothelial activation , capillary leakage ) should also be taken into account when treating hypovolemia in the critically ill .
	manualset3
88362	1	399638	5	NULL	NULL	0	NULL	drug actions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , drug actions on psi appear to be correlated with previously reported effects on Ca2 + transportation rather than oxidative phosphorylation associated with rat heart mitochondria .
	manualset3
88363	2	399638	5	NULL	NULL	0	NULL	psi	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , drug actions on psi appear to be correlated with previously reported effects on Ca2 + transportation rather than oxidative phosphorylation associated with rat heart mitochondria .
	manualset3
88364	3	399638	5	NULL	NULL	0	NULL	previously reported effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , drug actions on psi appear to be correlated with previously reported effects on Ca2 + transportation rather than oxidative phosphorylation associated with rat heart mitochondria .
	manualset3
88366	4	399638	5	NULL	NULL	NULL	NULL	Ca2 + transportation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In general , drug actions on psi appear to be correlated with previously reported effects on Ca2 + transportation rather than oxidative phosphorylation associated with rat heart mitochondria .
	manualset3
88368	5	399638	5	NULL	NULL	0	NULL	oxidative phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , drug actions on psi appear to be correlated with previously reported effects on Ca2 + transportation rather than oxidative phosphorylation associated with rat heart mitochondria .
	manualset3
88369	6	399638	5	NULL	NULL	0	NULL	rat heart mitochondria	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , drug actions on psi appear to be correlated with previously reported effects on Ca2 + transportation rather than oxidative phosphorylation associated with rat heart mitochondria .
	manualset3
88370	1	399639	5	NULL	NULL	0	NULL	managed care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , managed care has resulted in greater access to basic behavioral health and community-based services for children and adolescents , though access to inpatient hospital care has been reduced .
	manualset3
88374	2	399639	5	NULL	NULL	NULL	NULL	access to basic behavioral health	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In general , managed care has resulted in greater access to basic behavioral health and community-based services for children and adolescents , though access to inpatient hospital care has been reduced .
	manualset3
88375	3	399639	5	NULL	NULL	0	NULL	community-based services	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , managed care has resulted in greater access to basic behavioral health and community-based services for children and adolescents , though access to inpatient hospital care has been reduced .
	manualset3
88376	4	399639	5	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , managed care has resulted in greater access to basic behavioral health and community-based services for children and adolescents , though access to inpatient hospital care has been reduced .
	manualset3
88377	5	399639	5	NULL	NULL	0	NULL	adolescents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , managed care has resulted in greater access to basic behavioral health and community-based services for children and adolescents , though access to inpatient hospital care has been reduced .
	manualset3
88378	6	399639	5	NULL	NULL	0	NULL	access to inpatient hospital care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , managed care has resulted in greater access to basic behavioral health and community-based services for children and adolescents , though access to inpatient hospital care has been reduced .
	manualset3
88380	1	399640	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , patients with higher level of ECP , ECP/Eo ratio , sIL-2R , sICAM-1 and with lower PC20H exhibited the higher risk of moderate asthma .
	manualset3
88381	2	399640	5	NULL	NULL	0	NULL	higher level of ECP , ECP/Eo ratio , sIL-2R , sICAM-1	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , patients with higher level of ECP , ECP/Eo ratio , sIL-2R , sICAM-1 and with lower PC20H exhibited the higher risk of moderate asthma .
	manualset3
88382	3	399640	5	NULL	NULL	0	NULL	lower PC20H	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , patients with higher level of ECP , ECP/Eo ratio , sIL-2R , sICAM-1 and with lower PC20H exhibited the higher risk of moderate asthma .
	manualset3
88383	4	399640	5	NULL	NULL	0	NULL	higher risk of moderate asthma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , patients with higher level of ECP , ECP/Eo ratio , sIL-2R , sICAM-1 and with lower PC20H exhibited the higher risk of moderate asthma .
	manualset3
88387	1	399641	5	NULL	NULL	0	NULL	Transpharyngeal anterior atlanto-axial spondylodesis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Transpharyngeal anterior atlanto-axial spondylodesis for old fractures of the odontoid process of the axis and compression of the spinal cord ) .
	manualset3
88395	2	399641	5	NULL	NULL	0	NULL	old fractures of the odontoid process of the axis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Transpharyngeal anterior atlanto-axial spondylodesis for old fractures of the odontoid process of the axis and compression of the spinal cord ) .
	manualset3
88396	3	399641	5	NULL	NULL	0	NULL	compression of the spinal cord	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Transpharyngeal anterior atlanto-axial spondylodesis for old fractures of the odontoid process of the axis and compression of the spinal cord ) .
	manualset3
88398	1	399642	5	NULL	NULL	0	NULL	physically abused children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , physically abused children reported greater fear than nonabused children in response to all forms of interadult anger .
	manualset3
88400	2	399642	5	NULL	NULL	0	NULL	greater fear	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , physically abused children reported greater fear than nonabused children in response to all forms of interadult anger .
	manualset3
88401	3	399642	5	NULL	NULL	0	NULL	nonabused children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , physically abused children reported greater fear than nonabused children in response to all forms of interadult anger .
	manualset3
88402	4	399642	5	NULL	NULL	0	NULL	response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , physically abused children reported greater fear than nonabused children in response to all forms of interadult anger .
	manualset3
88403	5	399642	5	NULL	NULL	NULL	NULL	all forms of interadult anger	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In general , physically abused children reported greater fear than nonabused children in response to all forms of interadult anger .
	manualset3
88404	1	399643	5	NULL	NULL	0	NULL	non-marketed benefits	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , such non-marketed benefits provided by the case-study region more than compensate for the costs of forest maintenance .
	manualset3
88405	2	399643	5	NULL	NULL	0	NULL	case-study region	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , such non-marketed benefits provided by the case-study region more than compensate for the costs of forest maintenance .
	manualset3
88406	3	399643	5	NULL	NULL	0	NULL	compensate	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , such non-marketed benefits provided by the case-study region more than compensate for the costs of forest maintenance .
	manualset3
88407	4	399643	5	NULL	NULL	0	NULL	costs	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , such non-marketed benefits provided by the case-study region more than compensate for the costs of forest maintenance .
	manualset3
88408	5	399643	5	NULL	NULL	0	NULL	forest maintenance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , such non-marketed benefits provided by the case-study region more than compensate for the costs of forest maintenance .
	manualset3
88409	1	399644	5	NULL	NULL	NULL	NULL	demographic factors	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In general , the association between demographic factors and current HCV infection status was strengthened by use of latent-class analysis that combined data for markers of HCV infection , when compared with results of logistic regression analysis for each marker separately .
	manualset3
88410	2	399644	5	NULL	NULL	0	NULL	current HCV infection status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , the association between demographic factors and current HCV infection status was strengthened by use of latent-class analysis that combined data for markers of HCV infection , when compared with results of logistic regression analysis for each marker separately .
	manualset3
88411	3	399644	5	NULL	NULL	0	NULL	latent-class analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , the association between demographic factors and current HCV infection status was strengthened by use of latent-class analysis that combined data for markers of HCV infection , when compared with results of logistic regression analysis for each marker separately .
	manualset3
88412	4	399644	5	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , the association between demographic factors and current HCV infection status was strengthened by use of latent-class analysis that combined data for markers of HCV infection , when compared with results of logistic regression analysis for each marker separately .
	manualset3
88413	5	399644	5	NULL	NULL	0	NULL	markers of HCV infection	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , the association between demographic factors and current HCV infection status was strengthened by use of latent-class analysis that combined data for markers of HCV infection , when compared with results of logistic regression analysis for each marker separately .
	manualset3
88414	6	399644	5	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , the association between demographic factors and current HCV infection status was strengthened by use of latent-class analysis that combined data for markers of HCV infection , when compared with results of logistic regression analysis for each marker separately .
	manualset3
88415	7	399644	5	NULL	NULL	0	NULL	logistic regression analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , the association between demographic factors and current HCV infection status was strengthened by use of latent-class analysis that combined data for markers of HCV infection , when compared with results of logistic regression analysis for each marker separately .
	manualset3
88416	8	399644	5	NULL	NULL	0	NULL	marker	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , the association between demographic factors and current HCV infection status was strengthened by use of latent-class analysis that combined data for markers of HCV infection , when compared with results of logistic regression analysis for each marker separately .
	manualset3
88417	1	399645	5	NULL	NULL	0	NULL	Surgipro sutures	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , the new Surgipro sutures performed as good as Prolene sutures in terms of mechanical properties ; but there were some differences in fundamental properties between these two types of PP sutures , particularly in finer size PP sutures .
	manualset3
88418	2	399645	5	NULL	NULL	0	NULL	Prolene sutures	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , the new Surgipro sutures performed as good as Prolene sutures in terms of mechanical properties ; but there were some differences in fundamental properties between these two types of PP sutures , particularly in finer size PP sutures .
	manualset3
88419	3	399645	5	NULL	NULL	NULL	NULL	PP sutures	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In general , the new Surgipro sutures performed as good as Prolene sutures in terms of mechanical properties ; but there were some differences in fundamental properties between these two types of PP sutures , particularly in finer size PP sutures .
	manualset3
88420	4	399645	5	NULL	NULL	0	NULL	finer size PP sutures	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , the new Surgipro sutures performed as good as Prolene sutures in terms of mechanical properties ; but there were some differences in fundamental properties between these two types of PP sutures , particularly in finer size PP sutures .
	manualset3
88421	1	399646	5	NULL	NULL	0	NULL	goldfish	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In goldfish , unlike most teleosts , the vagal lobe is laminated , highly differentiated structure containing both sensory and motor layers .
	manualset3
88422	2	399646	5	NULL	NULL	0	NULL	teleosts	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In goldfish , unlike most teleosts , the vagal lobe is laminated , highly differentiated structure containing both sensory and motor layers .
	manualset3
88432	3	399646	5	NULL	NULL	0	NULL	vagal lobe	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In goldfish , unlike most teleosts , the vagal lobe is laminated , highly differentiated structure containing both sensory and motor layers .
	manualset3
88438	4	399646	5	NULL	NULL	0	NULL	sensory and motor layers	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In goldfish , unlike most teleosts , the vagal lobe is laminated , highly differentiated structure containing both sensory and motor layers .
	manualset3
88439	1	399647	5	NULL	NULL	0	NULL	hamsters	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In hamsters , tocopherols were the only tocol readily detected in all tissues , except adipose during tocotrienol supplementation .
	manualset3
88440	2	399647	5	NULL	NULL	0	NULL	tocopherols	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In hamsters , tocopherols were the only tocol readily detected in all tissues , except adipose during tocotrienol supplementation .
	manualset3
88442	3	399647	5	NULL	NULL	0	NULL	tocol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In hamsters , tocopherols were the only tocol readily detected in all tissues , except adipose during tocotrienol supplementation .
	manualset3
88443	4	399647	5	NULL	NULL	0	NULL	tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In hamsters , tocopherols were the only tocol readily detected in all tissues , except adipose during tocotrienol supplementation .
	manualset3
88444	5	399647	5	NULL	NULL	0	NULL	adipose	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In hamsters , tocopherols were the only tocol readily detected in all tissues , except adipose during tocotrienol supplementation .
	manualset3
88458	6	399647	5	NULL	NULL	NULL	NULL	tocotrienol supplementation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In hamsters , tocopherols were the only tocol readily detected in all tissues , except adipose during tocotrienol supplementation .
	manualset3
88459	1	399648	5	NULL	NULL	0	NULL	heart	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In heart , LDH-1 ( H4 ) was concentrated in mitochondria whereas LDH-5 ( M4 ) was present in both mitochondria and surrounding cytosol and organelles .
	manualset3
88460	2	399648	5	NULL	NULL	0	NULL	 LDH-1 ( H4 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In heart , LDH-1 ( H4 ) was concentrated in mitochondria whereas LDH-5 ( M4 ) was present in both mitochondria and surrounding cytosol and organelles .
	manualset3
88461	3	399648	5	NULL	NULL	0	NULL	mitochondria	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In heart , LDH-1 ( H4 ) was concentrated in mitochondria whereas LDH-5 ( M4 ) was present in both mitochondria and surrounding cytosol and organelles .
	manualset3
88462	4	399648	5	NULL	NULL	0	NULL	LDH-5 ( M4 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In heart , LDH-1 ( H4 ) was concentrated in mitochondria whereas LDH-5 ( M4 ) was present in both mitochondria and surrounding cytosol and organelles .
	manualset3
88463	5	399648	5	NULL	NULL	0	NULL	mitochondria	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In heart , LDH-1 ( H4 ) was concentrated in mitochondria whereas LDH-5 ( M4 ) was present in both mitochondria and surrounding cytosol and organelles .
	manualset3
88464	6	399648	5	NULL	NULL	0	NULL	surrounding cytosol and organelles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In heart , LDH-1 ( H4 ) was concentrated in mitochondria whereas LDH-5 ( M4 ) was present in both mitochondria and surrounding cytosol and organelles .
	manualset3
88465	1	399649	5	NULL	NULL	0	NULL	isolated , DNA synthesizing nuclei	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In isolated , DNA synthesizing nuclei , on the other hand , the slight inhibition of DNA synthesis by BTC is reversed merely by addition of Mg2 + .
	manualset3
88466	2	399649	5	NULL	NULL	0	NULL	slight inhibition of DNA synthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In isolated , DNA synthesizing nuclei , on the other hand , the slight inhibition of DNA synthesis by BTC is reversed merely by addition of Mg2 + .
	manualset3
88467	3	399649	5	NULL	NULL	0	NULL	BTC	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In isolated , DNA synthesizing nuclei , on the other hand , the slight inhibition of DNA synthesis by BTC is reversed merely by addition of Mg2 + .
	manualset3
88468	4	399649	5	NULL	NULL	NULL	NULL	addition of Mg2 +	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In isolated , DNA synthesizing nuclei , on the other hand , the slight inhibition of DNA synthesis by BTC is reversed merely by addition of Mg2 + .
	manualset3
88470	1	399650	5	NULL	NULL	0	NULL	males	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In males , Chlam Ab were not significantly related to the outcome of semen analysis , including screening for ASA ( IgG and/or IgA ) in semen , and several parameters of sperm functional capacity .
	manualset3
88471	2	399650	5	NULL	NULL	0	NULL	Chlam Ab	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In males , Chlam Ab were not significantly related to the outcome of semen analysis , including screening for ASA ( IgG and/or IgA ) in semen , and several parameters of sperm functional capacity .
	manualset3
88472	3	399650	5	NULL	NULL	0	NULL	outcome	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In males , Chlam Ab were not significantly related to the outcome of semen analysis , including screening for ASA ( IgG and/or IgA ) in semen , and several parameters of sperm functional capacity .
	manualset3
88473	4	399650	5	NULL	NULL	0	NULL	semen analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In males , Chlam Ab were not significantly related to the outcome of semen analysis , including screening for ASA ( IgG and/or IgA ) in semen , and several parameters of sperm functional capacity .
	manualset3
88474	5	399650	5	NULL	NULL	0	NULL	screening for ASA ( IgG and/or IgA )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In males , Chlam Ab were not significantly related to the outcome of semen analysis , including screening for ASA ( IgG and/or IgA ) in semen , and several parameters of sperm functional capacity .
	manualset3
88475	6	399650	5	NULL	NULL	NULL	NULL	semen	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In males , Chlam Ab were not significantly related to the outcome of semen analysis , including screening for ASA ( IgG and/or IgA ) in semen , and several parameters of sperm functional capacity .
	manualset3
88476	7	399650	5	NULL	NULL	0	NULL	several parameters	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In males , Chlam Ab were not significantly related to the outcome of semen analysis , including screening for ASA ( IgG and/or IgA ) in semen , and several parameters of sperm functional capacity .
	manualset3
88477	8	399650	5	NULL	NULL	0	NULL	sperm functional capacity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In males , Chlam Ab were not significantly related to the outcome of semen analysis , including screening for ASA ( IgG and/or IgA ) in semen , and several parameters of sperm functional capacity .
	manualset3
88483	1	399651	5	NULL	NULL	0	NULL	males	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In males , higher BR was observed in childhood-adolescence age groups and at older ages , while in females a higher level of BR was observed during childhood .
	manualset3
88492	2	399651	5	NULL	NULL	0	NULL	higher BR	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In males , higher BR was observed in childhood-adolescence age groups and at older ages , while in females a higher level of BR was observed during childhood .
	manualset3
88493	3	399651	5	NULL	NULL	0	NULL	childhood-adolescence age groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In males , higher BR was observed in childhood-adolescence age groups and at older ages , while in females a higher level of BR was observed during childhood .
	manualset3
88498	4	399651	5	NULL	NULL	0	NULL	older ages	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In males , higher BR was observed in childhood-adolescence age groups and at older ages , while in females a higher level of BR was observed during childhood .
	manualset3
88500	5	399651	5	NULL	NULL	0	NULL	females	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In males , higher BR was observed in childhood-adolescence age groups and at older ages , while in females a higher level of BR was observed during childhood .
	manualset3
88502	6	399651	5	NULL	NULL	0	NULL	higher level of BR	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In males , higher BR was observed in childhood-adolescence age groups and at older ages , while in females a higher level of BR was observed during childhood .
	manualset3
88506	7	399651	5	NULL	NULL	0	NULL	childhood	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In males , higher BR was observed in childhood-adolescence age groups and at older ages , while in females a higher level of BR was observed during childhood .
	manualset3
88507	1	399652	5	NULL	NULL	0	NULL	males	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In males , neither a history of a previous primary nor a history of radiotherapy was associated significantly with lung cancer ; however , the numbers of exposed cases were small .
	manualset3
88508	2	399652	5	NULL	NULL	0	NULL	history	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In males , neither a history of a previous primary nor a history of radiotherapy was associated significantly with lung cancer ; however , the numbers of exposed cases were small .
	manualset3
88509	3	399652	5	NULL	NULL	0	NULL	history	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In males , neither a history of a previous primary nor a history of radiotherapy was associated significantly with lung cancer ; however , the numbers of exposed cases were small .
	manualset3
88510	4	399652	5	NULL	NULL	0	NULL	radiotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In males , neither a history of a previous primary nor a history of radiotherapy was associated significantly with lung cancer ; however , the numbers of exposed cases were small .
	manualset3
88513	5	399652	5	NULL	NULL	0	NULL	lung cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In males , neither a history of a previous primary nor a history of radiotherapy was associated significantly with lung cancer ; however , the numbers of exposed cases were small .
	manualset3
88515	6	399652	5	NULL	NULL	0	NULL	numbers of exposed cases	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In males , neither a history of a previous primary nor a history of radiotherapy was associated significantly with lung cancer ; however , the numbers of exposed cases were small .
	manualset3
88518	1	399653	5	NULL	NULL	0	NULL	mammals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In mammals , imprinted genes directly regulate placental function and nutrient distribution from mother to fetus ; however , none of the & gt ; 60 imprinted genes thus far reported in plants have been demonstrated to play an equivalent role in regulating the flow of resources to the embryo .
	manualset3
88520	2	399653	5	NULL	NULL	0	NULL	imprinted genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In mammals , imprinted genes directly regulate placental function and nutrient distribution from mother to fetus ; however , none of the & gt ; 60 imprinted genes thus far reported in plants have been demonstrated to play an equivalent role in regulating the flow of resources to the embryo .
	manualset3
88521	3	399653	5	NULL	NULL	0	NULL	regulate placental function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In mammals , imprinted genes directly regulate placental function and nutrient distribution from mother to fetus ; however , none of the & gt ; 60 imprinted genes thus far reported in plants have been demonstrated to play an equivalent role in regulating the flow of resources to the embryo .
	manualset3
88522	4	399653	5	NULL	NULL	0	NULL	nutrient distribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In mammals , imprinted genes directly regulate placental function and nutrient distribution from mother to fetus ; however , none of the & gt ; 60 imprinted genes thus far reported in plants have been demonstrated to play an equivalent role in regulating the flow of resources to the embryo .
	manualset3
88525	5	399653	5	NULL	NULL	0	NULL	mother	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In mammals , imprinted genes directly regulate placental function and nutrient distribution from mother to fetus ; however , none of the & gt ; 60 imprinted genes thus far reported in plants have been demonstrated to play an equivalent role in regulating the flow of resources to the embryo .
	manualset3
88527	6	399653	5	NULL	NULL	0	NULL	fetus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In mammals , imprinted genes directly regulate placental function and nutrient distribution from mother to fetus ; however , none of the & gt ; 60 imprinted genes thus far reported in plants have been demonstrated to play an equivalent role in regulating the flow of resources to the embryo .
	manualset3
88530	7	399653	5	NULL	NULL	0	NULL	60 imprinted genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In mammals , imprinted genes directly regulate placental function and nutrient distribution from mother to fetus ; however , none of the & gt ; 60 imprinted genes thus far reported in plants have been demonstrated to play an equivalent role in regulating the flow of resources to the embryo .
	manualset3
88531	8	399653	5	NULL	NULL	0	NULL	plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In mammals , imprinted genes directly regulate placental function and nutrient distribution from mother to fetus ; however , none of the & gt ; 60 imprinted genes thus far reported in plants have been demonstrated to play an equivalent role in regulating the flow of resources to the embryo .
	manualset3
88532	9	399653	5	NULL	NULL	0	NULL	equivalent role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In mammals , imprinted genes directly regulate placental function and nutrient distribution from mother to fetus ; however , none of the & gt ; 60 imprinted genes thus far reported in plants have been demonstrated to play an equivalent role in regulating the flow of resources to the embryo .
	manualset3
88533	10	399653	5	NULL	NULL	0	NULL	flow of resources	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In mammals , imprinted genes directly regulate placental function and nutrient distribution from mother to fetus ; however , none of the & gt ; 60 imprinted genes thus far reported in plants have been demonstrated to play an equivalent role in regulating the flow of resources to the embryo .
	manualset3
88534	11	399653	5	NULL	NULL	0	NULL	embryo	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In mammals , imprinted genes directly regulate placental function and nutrient distribution from mother to fetus ; however , none of the & gt ; 60 imprinted genes thus far reported in plants have been demonstrated to play an equivalent role in regulating the flow of resources to the embryo .
	manualset3
88535	1	399654	5	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In men , the average length was 2.2 cm ( range 1.4-3 .8 cm ) , whereas in women the average length was 2.0 cm ( range 1.0-3 .2 cm ) ( P less than .01 ) .
	manualset3
88536	2	399654	5	NULL	NULL	0	NULL	average length	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In men , the average length was 2.2 cm ( range 1.4-3 .8 cm ) , whereas in women the average length was 2.0 cm ( range 1.0-3 .2 cm ) ( P less than .01 ) .
	manualset3
88537	3	399654	5	NULL	NULL	0	NULL	2.2 cm ( range 1.4-3 .8 cm )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In men , the average length was 2.2 cm ( range 1.4-3 .8 cm ) , whereas in women the average length was 2.0 cm ( range 1.0-3 .2 cm ) ( P less than .01 ) .
	manualset3
88538	4	399654	5	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In men , the average length was 2.2 cm ( range 1.4-3 .8 cm ) , whereas in women the average length was 2.0 cm ( range 1.0-3 .2 cm ) ( P less than .01 ) .
	manualset3
88539	5	399654	5	NULL	NULL	0	NULL	average length	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In men , the average length was 2.2 cm ( range 1.4-3 .8 cm ) , whereas in women the average length was 2.0 cm ( range 1.0-3 .2 cm ) ( P less than .01 ) .
	manualset3
88540	6	399654	5	NULL	NULL	0	NULL	2.0 cm ( range 1.0-3 .2 cm ) ( P less than .01 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In men , the average length was 2.2 cm ( range 1.4-3 .8 cm ) , whereas in women the average length was 2.0 cm ( range 1.0-3 .2 cm ) ( P less than .01 ) .
	manualset3
88541	1	399655	5	NULL	NULL	0	NULL	monkeys	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In monkeys , the selective KOR antagonist , nor-binaltorphimine ( nor-BNI ) , produces a long-lasting antagonism of the antinociceptive effects of U-50488H but not those of bremazocine , suggesting that KOR-mediated antinociception may occur through two distinct KORs .
	manualset3
88543	2	399655	5	NULL	NULL	0	NULL	selective KOR antagonist , nor-binaltorphimine ( nor-BNI )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In monkeys , the selective KOR antagonist , nor-binaltorphimine ( nor-BNI ) , produces a long-lasting antagonism of the antinociceptive effects of U-50488H but not those of bremazocine , suggesting that KOR-mediated antinociception may occur through two distinct KORs .
	manualset3
88545	3	399655	5	NULL	NULL	0	NULL	long-lasting antagonism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In monkeys , the selective KOR antagonist , nor-binaltorphimine ( nor-BNI ) , produces a long-lasting antagonism of the antinociceptive effects of U-50488H but not those of bremazocine , suggesting that KOR-mediated antinociception may occur through two distinct KORs .
	manualset3
88547	4	399655	5	NULL	NULL	0	NULL	antinociceptive effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In monkeys , the selective KOR antagonist , nor-binaltorphimine ( nor-BNI ) , produces a long-lasting antagonism of the antinociceptive effects of U-50488H but not those of bremazocine , suggesting that KOR-mediated antinociception may occur through two distinct KORs .
	manualset3
88551	5	399655	5	NULL	NULL	0	NULL	U-50488H 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In monkeys , the selective KOR antagonist , nor-binaltorphimine ( nor-BNI ) , produces a long-lasting antagonism of the antinociceptive effects of U-50488H but not those of bremazocine , suggesting that KOR-mediated antinociception may occur through two distinct KORs .
	manualset3
88633	6	399655	5	NULL	NULL	0	NULL	bremazocine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In monkeys , the selective KOR antagonist , nor-binaltorphimine ( nor-BNI ) , produces a long-lasting antagonism of the antinociceptive effects of U-50488H but not those of bremazocine , suggesting that KOR-mediated antinociception may occur through two distinct KORs .
	manualset3
88634	7	399655	5	NULL	NULL	0	NULL	KOR-mediated antinociception	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In monkeys , the selective KOR antagonist , nor-binaltorphimine ( nor-BNI ) , produces a long-lasting antagonism of the antinociceptive effects of U-50488H but not those of bremazocine , suggesting that KOR-mediated antinociception may occur through two distinct KORs .
	manualset3
88635	8	399655	5	NULL	NULL	0	NULL	KORs	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In monkeys , the selective KOR antagonist , nor-binaltorphimine ( nor-BNI ) , produces a long-lasting antagonism of the antinociceptive effects of U-50488H but not those of bremazocine , suggesting that KOR-mediated antinociception may occur through two distinct KORs .
	manualset3
88636	1	399656	5	NULL	NULL	NULL	NULL	Traumatic false aneurysm	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Traumatic false aneurysm of the superior mesenteric artery with perforation into the duodenum ; surgery ; recovery ) .
	manualset3
88637	2	399656	5	NULL	NULL	0	NULL	superior mesenteric artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Traumatic false aneurysm of the superior mesenteric artery with perforation into the duodenum ; surgery ; recovery ) .
	manualset3
88638	3	399656	5	NULL	NULL	0	NULL	perforation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Traumatic false aneurysm of the superior mesenteric artery with perforation into the duodenum ; surgery ; recovery ) .
	manualset3
88639	4	399656	5	NULL	NULL	0	NULL	duodenum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Traumatic false aneurysm of the superior mesenteric artery with perforation into the duodenum ; surgery ; recovery ) .
	manualset3
88640	5	399656	5	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Traumatic false aneurysm of the superior mesenteric artery with perforation into the duodenum ; surgery ; recovery ) .
	manualset3
88641	6	399656	5	NULL	NULL	0	NULL	recovery	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Traumatic false aneurysm of the superior mesenteric artery with perforation into the duodenum ; surgery ; recovery ) .
	manualset3
88642	1	399657	5	NULL	NULL	0	NULL	immunofluorescence study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In parallel , an immunofluorescence study of tight-junction protein expression of PND60 offspring from contaminated rats showed a disorganization of the tight-junction proteins claudin-2 and claudin-5 , specifically expressed in the proximal tubule and glomerulus , respectively .
	manualset3
88643	2	399657	5	NULL	NULL	NULL	NULL	tight-junction protein expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In parallel , an immunofluorescence study of tight-junction protein expression of PND60 offspring from contaminated rats showed a disorganization of the tight-junction proteins claudin-2 and claudin-5 , specifically expressed in the proximal tubule and glomerulus , respectively .
	manualset3
88644	3	399657	5	NULL	NULL	0	NULL	PND60 offspring	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In parallel , an immunofluorescence study of tight-junction protein expression of PND60 offspring from contaminated rats showed a disorganization of the tight-junction proteins claudin-2 and claudin-5 , specifically expressed in the proximal tubule and glomerulus , respectively .
	manualset3
88645	4	399657	5	NULL	NULL	0	NULL	contaminated rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In parallel , an immunofluorescence study of tight-junction protein expression of PND60 offspring from contaminated rats showed a disorganization of the tight-junction proteins claudin-2 and claudin-5 , specifically expressed in the proximal tubule and glomerulus , respectively .
	manualset3
88646	5	399657	5	NULL	NULL	0	NULL	disorganization of the tight-junction protein claudin-2	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In parallel , an immunofluorescence study of tight-junction protein expression of PND60 offspring from contaminated rats showed a disorganization of the tight-junction proteins claudin-2 and claudin-5 , specifically expressed in the proximal tubule and glomerulus , respectively .
	manualset3
88647	6	399657	5	NULL	NULL	0	NULL	disorganization of the tight-junction proteins claudin-5	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In parallel , an immunofluorescence study of tight-junction protein expression of PND60 offspring from contaminated rats showed a disorganization of the tight-junction proteins claudin-2 and claudin-5 , specifically expressed in the proximal tubule and glomerulus , respectively .
	manualset3
88648	7	399657	5	NULL	NULL	0	NULL	proximal tubule	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In parallel , an immunofluorescence study of tight-junction protein expression of PND60 offspring from contaminated rats showed a disorganization of the tight-junction proteins claudin-2 and claudin-5 , specifically expressed in the proximal tubule and glomerulus , respectively .
	manualset3
88649	8	399657	5	NULL	NULL	0	NULL	glomerulus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In parallel , an immunofluorescence study of tight-junction protein expression of PND60 offspring from contaminated rats showed a disorganization of the tight-junction proteins claudin-2 and claudin-5 , specifically expressed in the proximal tubule and glomerulus , respectively .
	manualset3
88650	1	399658	5	NULL	NULL	0	NULL	multigram-scale diastereoselective diacetoxylation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , a multigram-scale diastereoselective diacetoxylation of methyl cinnamate ( 5.00 g ) was also accomplished in a few hours , maintaining the same efficiency as small-scale reaction .
	manualset3
88651	2	399658	5	NULL	NULL	0	NULL	methyl cinnamate ( 5.00 g ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , a multigram-scale diastereoselective diacetoxylation of methyl cinnamate ( 5.00 g ) was also accomplished in a few hours , maintaining the same efficiency as small-scale reaction .
	manualset3
88652	3	399658	5	NULL	NULL	0	NULL	few hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , a multigram-scale diastereoselective diacetoxylation of methyl cinnamate ( 5.00 g ) was also accomplished in a few hours , maintaining the same efficiency as small-scale reaction .
	manualset3
88653	4	399658	5	NULL	NULL	0	NULL	efficiency	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , a multigram-scale diastereoselective diacetoxylation of methyl cinnamate ( 5.00 g ) was also accomplished in a few hours , maintaining the same efficiency as small-scale reaction .
	manualset3
88654	5	399658	5	NULL	NULL	0	NULL	small-scale reaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , a multigram-scale diastereoselective diacetoxylation of methyl cinnamate ( 5.00 g ) was also accomplished in a few hours , maintaining the same efficiency as small-scale reaction .
	manualset3
88655	1	399659	5	NULL	NULL	0	NULL	subgroup of NPY-I neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , a subgroup of NPY-I neurons , distinguished by a higher percentage of unmyelinated axon coverage of the plasmalemmal surface , was present in young , but not aged , rats .
	manualset3
88656	2	399659	5	NULL	NULL	0	NULL	higher percentage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , a subgroup of NPY-I neurons , distinguished by a higher percentage of unmyelinated axon coverage of the plasmalemmal surface , was present in young , but not aged , rats .
	manualset3
88657	3	399659	5	NULL	NULL	0	NULL	unmyelinated axon coverage of the plasmalemmal surface	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , a subgroup of NPY-I neurons , distinguished by a higher percentage of unmyelinated axon coverage of the plasmalemmal surface , was present in young , but not aged , rats .
	manualset3
88658	4	399659	5	NULL	NULL	0	NULL	young rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , a subgroup of NPY-I neurons , distinguished by a higher percentage of unmyelinated axon coverage of the plasmalemmal surface , was present in young , but not aged , rats .
	manualset3
88659	5	399659	5	NULL	NULL	0	NULL	aged , rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , a subgroup of NPY-I neurons , distinguished by a higher percentage of unmyelinated axon coverage of the plasmalemmal surface , was present in young , but not aged , rats .
	manualset3
88660	1	399660	5	NULL	NULL	0	NULL	accidental wounds	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , accidental wounds produced by used needles , especially needles contaminated with blood from Ag H be positive individuals , are frequently followed by clinical or serological evidence of viral hepatitis .
	manualset3
88661	2	399660	5	NULL	NULL	0	NULL	used needles	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , accidental wounds produced by used needles , especially needles contaminated with blood from Ag H be positive individuals , are frequently followed by clinical or serological evidence of viral hepatitis .
	manualset3
88662	3	399660	5	NULL	NULL	0	NULL	 needles	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , accidental wounds produced by used needles , especially needles contaminated with blood from Ag H be positive individuals , are frequently followed by clinical or serological evidence of viral hepatitis .
	manualset3
88663	4	399660	5	NULL	NULL	0	NULL	blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , accidental wounds produced by used needles , especially needles contaminated with blood from Ag H be positive individuals , are frequently followed by clinical or serological evidence of viral hepatitis .
	manualset3
88664	5	399660	5	NULL	NULL	0	NULL	Ag H be positive individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , accidental wounds produced by used needles , especially needles contaminated with blood from Ag H be positive individuals , are frequently followed by clinical or serological evidence of viral hepatitis .
	manualset3
88665	6	399660	5	NULL	NULL	0	NULL	clinical or serological evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , accidental wounds produced by used needles , especially needles contaminated with blood from Ag H be positive individuals , are frequently followed by clinical or serological evidence of viral hepatitis .
	manualset3
88666	7	399660	5	NULL	NULL	0	NULL	viral hepatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , accidental wounds produced by used needles , especially needles contaminated with blood from Ag H be positive individuals , are frequently followed by clinical or serological evidence of viral hepatitis .
	manualset3
88667	1	399661	5	NULL	NULL	0	NULL	pharmacological studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , pharmacological studies highlighted the crucial role for the neuropeptide oxytocin in social behavior and emotional perception .
	manualset3
88668	2	399661	5	NULL	NULL	0	NULL	crucial role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , pharmacological studies highlighted the crucial role for the neuropeptide oxytocin in social behavior and emotional perception .
	manualset3
88669	3	399661	5	NULL	NULL	0	NULL	neuropeptide oxytocin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , pharmacological studies highlighted the crucial role for the neuropeptide oxytocin in social behavior and emotional perception .
	manualset3
88670	4	399661	5	NULL	NULL	0	NULL	social behavior	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , pharmacological studies highlighted the crucial role for the neuropeptide oxytocin in social behavior and emotional perception .
	manualset3
88671	5	399661	5	NULL	NULL	0	NULL	emotional perception	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , pharmacological studies highlighted the crucial role for the neuropeptide oxytocin in social behavior and emotional perception .
	manualset3
88672	1	399662	5	NULL	NULL	0	NULL	phylogenetic methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , phylogenetic methods can quantitatively ( 1 ) test whether specific cognitive abilities are correlated with life history ( e.g. , lifespan ) , morphology ( e.g. , brain size ) , or socio-ecological variables ( e.g. , social system ) , ( 2 ) measure how strongly phylogenetic relatedness predicts the distribution of cognitive skills across species , and ( 3 ) estimate the ancestral state of a given cognitive trait using measures of cognitive performance from extant species .
	manualset3
88674	2	399662	5	NULL	NULL	NULL	NULL	specific cognitive abilities	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In particular , phylogenetic methods can quantitatively ( 1 ) test whether specific cognitive abilities are correlated with life history ( e.g. , lifespan ) , morphology ( e.g. , brain size ) , or socio-ecological variables ( e.g. , social system ) , ( 2 ) measure how strongly phylogenetic relatedness predicts the distribution of cognitive skills across species , and ( 3 ) estimate the ancestral state of a given cognitive trait using measures of cognitive performance from extant species .
	manualset3
88675	3	399662	5	NULL	NULL	NULL	NULL	life history ( e.g. , lifespan )	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In particular , phylogenetic methods can quantitatively ( 1 ) test whether specific cognitive abilities are correlated with life history ( e.g. , lifespan ) , morphology ( e.g. , brain size ) , or socio-ecological variables ( e.g. , social system ) , ( 2 ) measure how strongly phylogenetic relatedness predicts the distribution of cognitive skills across species , and ( 3 ) estimate the ancestral state of a given cognitive trait using measures of cognitive performance from extant species .
	manualset3
88676	4	399662	5	NULL	NULL	NULL	NULL	morphology ( e.g. , brain size )	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In particular , phylogenetic methods can quantitatively ( 1 ) test whether specific cognitive abilities are correlated with life history ( e.g. , lifespan ) , morphology ( e.g. , brain size ) , or socio-ecological variables ( e.g. , social system ) , ( 2 ) measure how strongly phylogenetic relatedness predicts the distribution of cognitive skills across species , and ( 3 ) estimate the ancestral state of a given cognitive trait using measures of cognitive performance from extant species .
	manualset3
88677	5	399662	5	NULL	NULL	NULL	NULL	socio-ecological variables ( e.g. , social system )	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In particular , phylogenetic methods can quantitatively ( 1 ) test whether specific cognitive abilities are correlated with life history ( e.g. , lifespan ) , morphology ( e.g. , brain size ) , or socio-ecological variables ( e.g. , social system ) , ( 2 ) measure how strongly phylogenetic relatedness predicts the distribution of cognitive skills across species , and ( 3 ) estimate the ancestral state of a given cognitive trait using measures of cognitive performance from extant species .
	manualset3
88679	6	399662	5	NULL	NULL	NULL	NULL	phylogenetic relatedness	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In particular , phylogenetic methods can quantitatively ( 1 ) test whether specific cognitive abilities are correlated with life history ( e.g. , lifespan ) , morphology ( e.g. , brain size ) , or socio-ecological variables ( e.g. , social system ) , ( 2 ) measure how strongly phylogenetic relatedness predicts the distribution of cognitive skills across species , and ( 3 ) estimate the ancestral state of a given cognitive trait using measures of cognitive performance from extant species .
	manualset3
88680	9	399662	5	NULL	NULL	0	NULL	distribution of cognitive skills	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , phylogenetic methods can quantitatively ( 1 ) test whether specific cognitive abilities are correlated with life history ( e.g. , lifespan ) , morphology ( e.g. , brain size ) , or socio-ecological variables ( e.g. , social system ) , ( 2 ) measure how strongly phylogenetic relatedness predicts the distribution of cognitive skills across species , and ( 3 ) estimate the ancestral state of a given cognitive trait using measures of cognitive performance from extant species .
	manualset3
88681	10	399662	5	NULL	NULL	0	NULL	species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , phylogenetic methods can quantitatively ( 1 ) test whether specific cognitive abilities are correlated with life history ( e.g. , lifespan ) , morphology ( e.g. , brain size ) , or socio-ecological variables ( e.g. , social system ) , ( 2 ) measure how strongly phylogenetic relatedness predicts the distribution of cognitive skills across species , and ( 3 ) estimate the ancestral state of a given cognitive trait using measures of cognitive performance from extant species .
	manualset3
88683	11	399662	5	NULL	NULL	NULL	NULL	ancestral state	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In particular , phylogenetic methods can quantitatively ( 1 ) test whether specific cognitive abilities are correlated with life history ( e.g. , lifespan ) , morphology ( e.g. , brain size ) , or socio-ecological variables ( e.g. , social system ) , ( 2 ) measure how strongly phylogenetic relatedness predicts the distribution of cognitive skills across species , and ( 3 ) estimate the ancestral state of a given cognitive trait using measures of cognitive performance from extant species .
	manualset3
88684	12	399662	5	NULL	NULL	NULL	NULL	cognitive trait	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In particular , phylogenetic methods can quantitatively ( 1 ) test whether specific cognitive abilities are correlated with life history ( e.g. , lifespan ) , morphology ( e.g. , brain size ) , or socio-ecological variables ( e.g. , social system ) , ( 2 ) measure how strongly phylogenetic relatedness predicts the distribution of cognitive skills across species , and ( 3 ) estimate the ancestral state of a given cognitive trait using measures of cognitive performance from extant species .
	manualset3
88685	13	399662	5	NULL	NULL	NULL	NULL	cognitive performance	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In particular , phylogenetic methods can quantitatively ( 1 ) test whether specific cognitive abilities are correlated with life history ( e.g. , lifespan ) , morphology ( e.g. , brain size ) , or socio-ecological variables ( e.g. , social system ) , ( 2 ) measure how strongly phylogenetic relatedness predicts the distribution of cognitive skills across species , and ( 3 ) estimate the ancestral state of a given cognitive trait using measures of cognitive performance from extant species .
	manualset3
88686	14	399662	5	NULL	NULL	NULL	NULL	extant species	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In particular , phylogenetic methods can quantitatively ( 1 ) test whether specific cognitive abilities are correlated with life history ( e.g. , lifespan ) , morphology ( e.g. , brain size ) , or socio-ecological variables ( e.g. , social system ) , ( 2 ) measure how strongly phylogenetic relatedness predicts the distribution of cognitive skills across species , and ( 3 ) estimate the ancestral state of a given cognitive trait using measures of cognitive performance from extant species .
	manualset3
88687	1	399663	5	NULL	NULL	0	NULL	examples	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , some examples such as the selective determination of inorganic and metallorganic species of different toxicity and the redox state speciation of multiply charged ions are discussed .
	manualset3
88688	2	399663	5	NULL	NULL	0	NULL	selective determination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , some examples such as the selective determination of inorganic and metallorganic species of different toxicity and the redox state speciation of multiply charged ions are discussed .
	manualset3
88689	3	399663	5	NULL	NULL	0	NULL	inorganic and metallorganic species	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , some examples such as the selective determination of inorganic and metallorganic species of different toxicity and the redox state speciation of multiply charged ions are discussed .
	manualset3
88690	4	399663	5	NULL	NULL	0	NULL	toxicity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , some examples such as the selective determination of inorganic and metallorganic species of different toxicity and the redox state speciation of multiply charged ions are discussed .
	manualset3
88691	5	399663	5	NULL	NULL	NULL	NULL	redox state speciation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In particular , some examples such as the selective determination of inorganic and metallorganic species of different toxicity and the redox state speciation of multiply charged ions are discussed .
	manualset3
88692	6	399663	5	NULL	NULL	0	NULL	multiply charged ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , some examples such as the selective determination of inorganic and metallorganic species of different toxicity and the redox state speciation of multiply charged ions are discussed .
	manualset3
88693	1	399664	5	NULL	NULL	0	NULL	EHHST	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , the EHHST facilitates the computation of an asymptotic P-value instead of an empirical P-value , using simulations .
	manualset3
88694	2	399664	5	NULL	NULL	0	NULL	computation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , the EHHST facilitates the computation of an asymptotic P-value instead of an empirical P-value , using simulations .
	manualset3
88695	3	399664	5	NULL	NULL	0	NULL	asymptotic P-value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , the EHHST facilitates the computation of an asymptotic P-value instead of an empirical P-value , using simulations .
	manualset3
88696	4	399664	5	NULL	NULL	0	NULL	empirical P-value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , the EHHST facilitates the computation of an asymptotic P-value instead of an empirical P-value , using simulations .
	manualset3
88697	5	399664	5	NULL	NULL	NULL	NULL	simulations	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In particular , the EHHST facilitates the computation of an asymptotic P-value instead of an empirical P-value , using simulations .
	manualset3
88698	1	399665	5	NULL	NULL	0	NULL	engineering	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , the engineering of redox relays between roGFPs and redox enzymes allows control of probe specificity and enhancement of sensitivity .
	manualset3
88699	2	399665	5	NULL	NULL	NULL	NULL	redox relays	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In particular , the engineering of redox relays between roGFPs and redox enzymes allows control of probe specificity and enhancement of sensitivity .
	manualset3
88700	3	399665	5	NULL	NULL	0	NULL	roGFPs	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , the engineering of redox relays between roGFPs and redox enzymes allows control of probe specificity and enhancement of sensitivity .
	manualset3
88701	4	399665	5	NULL	NULL	0	NULL	redox enzymes	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , the engineering of redox relays between roGFPs and redox enzymes allows control of probe specificity and enhancement of sensitivity .
	manualset3
88702	5	399665	5	NULL	NULL	NULL	NULL	control of probe specificity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In particular , the engineering of redox relays between roGFPs and redox enzymes allows control of probe specificity and enhancement of sensitivity .
	manualset3
88703	6	399665	5	NULL	NULL	0	NULL	enhancement of sensitivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , the engineering of redox relays between roGFPs and redox enzymes allows control of probe specificity and enhancement of sensitivity .
	manualset3
88704	1	399666	5	NULL	NULL	0	NULL	focus	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , the focus is on the unique properties of peptide selection by I-Ag7 that reveal the preferred binding motif of diabetogenic MHC molecules and its role in display of peptides derived from islet beta cells .
	manualset3
88705	2	399666	5	NULL	NULL	0	NULL	unique properties of peptide selection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , the focus is on the unique properties of peptide selection by I-Ag7 that reveal the preferred binding motif of diabetogenic MHC molecules and its role in display of peptides derived from islet beta cells .
	manualset3
88706	3	399666	5	NULL	NULL	0	NULL	I-Ag7	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , the focus is on the unique properties of peptide selection by I-Ag7 that reveal the preferred binding motif of diabetogenic MHC molecules and its role in display of peptides derived from islet beta cells .
	manualset3
88707	4	399666	5	NULL	NULL	0	NULL	preferred binding motif	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , the focus is on the unique properties of peptide selection by I-Ag7 that reveal the preferred binding motif of diabetogenic MHC molecules and its role in display of peptides derived from islet beta cells .
	manualset3
88708	5	399666	5	NULL	NULL	0	NULL	diabetogenic MHC molecules	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , the focus is on the unique properties of peptide selection by I-Ag7 that reveal the preferred binding motif of diabetogenic MHC molecules and its role in display of peptides derived from islet beta cells .
	manualset3
88709	6	399666	5	NULL	NULL	0	NULL	 role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , the focus is on the unique properties of peptide selection by I-Ag7 that reveal the preferred binding motif of diabetogenic MHC molecules and its role in display of peptides derived from islet beta cells .
	manualset3
88710	7	399666	5	NULL	NULL	0	NULL	peptides derived from islet beta cells	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , the focus is on the unique properties of peptide selection by I-Ag7 that reveal the preferred binding motif of diabetogenic MHC molecules and its role in display of peptides derived from islet beta cells .
	manualset3
88711	1	399667	5	NULL	NULL	0	NULL	 high percentages of positive sheep sera	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , the high percentages of positive sheep sera in Martinique ( 15 % ) and Montserrat ( 11 % ) should be further investigated .
	manualset3
88712	2	399667	5	NULL	NULL	0	NULL	Martinique	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , the high percentages of positive sheep sera in Martinique ( 15 % ) and Montserrat ( 11 % ) should be further investigated .
	manualset3
88713	3	399667	5	NULL	NULL	0	NULL	15 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , the high percentages of positive sheep sera in Martinique ( 15 % ) and Montserrat ( 11 % ) should be further investigated .
	manualset3
88714	4	399667	5	NULL	NULL	0	NULL	Montserrat	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , the high percentages of positive sheep sera in Martinique ( 15 % ) and Montserrat ( 11 % ) should be further investigated .
	manualset3
88715	5	399667	5	NULL	NULL	0	NULL	11 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , the high percentages of positive sheep sera in Martinique ( 15 % ) and Montserrat ( 11 % ) should be further investigated .
	manualset3
88716	1	399668	5	NULL	NULL	NULL	NULL	substitution	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In particular , the substitution of Thr220 by serine is unique to Pr1B .
	manualset3
88717	2	399668	5	NULL	NULL	0	NULL	Thr220	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , the substitution of Thr220 by serine is unique to Pr1B .
	manualset3
88718	3	399668	5	NULL	NULL	0	NULL	serine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , the substitution of Thr220 by serine is unique to Pr1B .
	manualset3
88719	4	399668	5	NULL	NULL	0	NULL	Pr1B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , the substitution of Thr220 by serine is unique to Pr1B .
	manualset3
88720	1	399669	5	NULL	NULL	0	NULL	signal-to-noise ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , to increase the signal-to-noise ratio and to mitigate the adverse effect of residual image misalignments , DTI data are often smoothed before VBA with an isotropic Gaussian kernel with a full width half maximum up to 16 x 16 x 16 mm ( 3 ) .
	manualset3
88721	2	399669	5	NULL	NULL	NULL	NULL	adverse effect	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In particular , to increase the signal-to-noise ratio and to mitigate the adverse effect of residual image misalignments , DTI data are often smoothed before VBA with an isotropic Gaussian kernel with a full width half maximum up to 16 x 16 x 16 mm ( 3 ) .
	manualset3
88722	3	399669	5	NULL	NULL	0	NULL	residual image misalignments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , to increase the signal-to-noise ratio and to mitigate the adverse effect of residual image misalignments , DTI data are often smoothed before VBA with an isotropic Gaussian kernel with a full width half maximum up to 16 x 16 x 16 mm ( 3 ) .
	manualset3
88723	4	399669	5	NULL	NULL	0	NULL	DTI data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , to increase the signal-to-noise ratio and to mitigate the adverse effect of residual image misalignments , DTI data are often smoothed before VBA with an isotropic Gaussian kernel with a full width half maximum up to 16 x 16 x 16 mm ( 3 ) .
	manualset3
88724	5	399669	5	NULL	NULL	NULL	NULL	VBA	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In particular , to increase the signal-to-noise ratio and to mitigate the adverse effect of residual image misalignments , DTI data are often smoothed before VBA with an isotropic Gaussian kernel with a full width half maximum up to 16 x 16 x 16 mm ( 3 ) .
	manualset3
88725	6	399669	5	NULL	NULL	NULL	NULL	isotropic Gaussian kernel	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In particular , to increase the signal-to-noise ratio and to mitigate the adverse effect of residual image misalignments , DTI data are often smoothed before VBA with an isotropic Gaussian kernel with a full width half maximum up to 16 x 16 x 16 mm ( 3 ) .
	manualset3
88726	7	399669	5	NULL	NULL	0	NULL	full width half maximum up to 16 x 16 x 16 mm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , to increase the signal-to-noise ratio and to mitigate the adverse effect of residual image misalignments , DTI data are often smoothed before VBA with an isotropic Gaussian kernel with a full width half maximum up to 16 x 16 x 16 mm ( 3 ) .
	manualset3
88727	1	399670	5	NULL	NULL	0	NULL	photoreceptors 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In photoreceptors , targeted toxin expression results in increased Fasciclin II and chaoptin but not IrreC-rst immunoreactivity .
	manualset3
88728	2	399670	5	NULL	NULL	0	NULL	targeted toxin expression	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In photoreceptors , targeted toxin expression results in increased Fasciclin II and chaoptin but not IrreC-rst immunoreactivity .
	manualset3
88729	3	399670	5	NULL	NULL	0	NULL	Fasciclin II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In photoreceptors , targeted toxin expression results in increased Fasciclin II and chaoptin but not IrreC-rst immunoreactivity .
	manualset3
88730	4	399670	5	NULL	NULL	0	NULL	chaoptin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In photoreceptors , targeted toxin expression results in increased Fasciclin II and chaoptin but not IrreC-rst immunoreactivity .
	manualset3
88731	5	399670	5	NULL	NULL	0	NULL	IrreC-rst immunoreactivity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In photoreceptors , targeted toxin expression results in increased Fasciclin II and chaoptin but not IrreC-rst immunoreactivity .
	manualset3
88732	1	399671	5	NULL	NULL	0	NULL	plastids	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In plastids , at least six assembly factors are required for heme attachment to the apo-forms of cytochrome f and cytochrome c ( 6 ) in the thylakoid lumen .
	manualset3
88733	2	399671	5	NULL	NULL	0	NULL	six assembly factors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In plastids , at least six assembly factors are required for heme attachment to the apo-forms of cytochrome f and cytochrome c ( 6 ) in the thylakoid lumen .
	manualset3
88734	3	399671	5	NULL	NULL	0	NULL	heme attachment	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In plastids , at least six assembly factors are required for heme attachment to the apo-forms of cytochrome f and cytochrome c ( 6 ) in the thylakoid lumen .
	manualset3
88735	4	399671	5	NULL	NULL	0	NULL	apo-forms of cytochrome f and cytochrome c	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In plastids , at least six assembly factors are required for heme attachment to the apo-forms of cytochrome f and cytochrome c ( 6 ) in the thylakoid lumen .
	manualset3
88736	5	399671	5	NULL	NULL	0	NULL	thylakoid lumen	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In plastids , at least six assembly factors are required for heme attachment to the apo-forms of cytochrome f and cytochrome c ( 6 ) in the thylakoid lumen .
	manualset3
88737	1	399672	5	NULL	NULL	0	NULL	scenario	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In principle , the scenario is prepared to make the most of this information for the analysis of the dynamics of signalling pathways .
	manualset3
88738	2	399672	5	NULL	NULL	0	NULL	information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In principle , the scenario is prepared to make the most of this information for the analysis of the dynamics of signalling pathways .
	manualset3
88739	3	399672	5	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In principle , the scenario is prepared to make the most of this information for the analysis of the dynamics of signalling pathways .
	manualset3
88740	4	399672	5	NULL	NULL	0	NULL	dynamics of signalling pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In principle , the scenario is prepared to make the most of this information for the analysis of the dynamics of signalling pathways .
	manualset3
88741	1	399673	5	NULL	NULL	0	NULL	rodents	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In rodents , a cognitive anti-aging effect of DHEA and DHEAS has been observed but it is unclear whether this effect is mediated indirectly through conversion of these steroids to estradiol .
	manualset3
88742	2	399673	5	NULL	NULL	0	NULL	cognitive anti-aging effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In rodents , a cognitive anti-aging effect of DHEA and DHEAS has been observed but it is unclear whether this effect is mediated indirectly through conversion of these steroids to estradiol .
	manualset3
88743	3	399673	5	NULL	NULL	0	NULL	DHEA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In rodents , a cognitive anti-aging effect of DHEA and DHEAS has been observed but it is unclear whether this effect is mediated indirectly through conversion of these steroids to estradiol .
	manualset3
88744	4	399673	5	NULL	NULL	0	NULL	DHEAS	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In rodents , a cognitive anti-aging effect of DHEA and DHEAS has been observed but it is unclear whether this effect is mediated indirectly through conversion of these steroids to estradiol .
	manualset3
88745	5	399673	5	NULL	NULL	0	NULL	effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In rodents , a cognitive anti-aging effect of DHEA and DHEAS has been observed but it is unclear whether this effect is mediated indirectly through conversion of these steroids to estradiol .
	manualset3
88746	6	399673	5	NULL	NULL	0	NULL	conversion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In rodents , a cognitive anti-aging effect of DHEA and DHEAS has been observed but it is unclear whether this effect is mediated indirectly through conversion of these steroids to estradiol .
	manualset3
88747	7	399673	5	NULL	NULL	NULL	NULL	steroids	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In rodents , a cognitive anti-aging effect of DHEA and DHEAS has been observed but it is unclear whether this effect is mediated indirectly through conversion of these steroids to estradiol .
	manualset3
88748	8	399673	5	NULL	NULL	0	NULL	estradiol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In rodents , a cognitive anti-aging effect of DHEA and DHEAS has been observed but it is unclear whether this effect is mediated indirectly through conversion of these steroids to estradiol .
	manualset3
88749	1	399674	5	NULL	NULL	0	NULL	serum	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In serum , most of the 125I-IGFBP-3 was in the 150 kDa fraction , while most 125I-IGFBP-3 in milk was in the 40 kDa fraction .
	manualset3
88750	2	399674	5	NULL	NULL	0	NULL	125I-IGFBP-3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In serum , most of the 125I-IGFBP-3 was in the 150 kDa fraction , while most 125I-IGFBP-3 in milk was in the 40 kDa fraction .
	manualset3
88751	3	399674	5	NULL	NULL	0	NULL	150 kDa fraction	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In serum , most of the 125I-IGFBP-3 was in the 150 kDa fraction , while most 125I-IGFBP-3 in milk was in the 40 kDa fraction .
	manualset3
88752	4	399674	5	NULL	NULL	0	NULL	125I-IGFBP-3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In serum , most of the 125I-IGFBP-3 was in the 150 kDa fraction , while most 125I-IGFBP-3 in milk was in the 40 kDa fraction .
	manualset3
88753	5	399674	5	NULL	NULL	0	NULL	milk	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	In serum , most of the 125I-IGFBP-3 was in the 150 kDa fraction , while most 125I-IGFBP-3 in milk was in the 40 kDa fraction .
	manualset3
88754	6	399674	5	NULL	NULL	0	NULL	40 kDa fraction	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In serum , most of the 125I-IGFBP-3 was in the 150 kDa fraction , while most 125I-IGFBP-3 in milk was in the 40 kDa fraction .
	manualset3
88755	1	399675	5	NULL	NULL	0	NULL	seven ( Group I )	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In seven ( Group I ) predominantly unilateral disease was discovered by angiography ( renal-artery stenosis in six and hydronephrosis in one ) ; in the remaining seven ( Group II ) no rennal-artery abnormality was found .
	manualset3
88756	2	399675	5	NULL	NULL	0	NULL	unilateral disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In seven ( Group I ) predominantly unilateral disease was discovered by angiography ( renal-artery stenosis in six and hydronephrosis in one ) ; in the remaining seven ( Group II ) no rennal-artery abnormality was found .
	manualset3
88757	3	399675	5	NULL	NULL	0	NULL	angiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In seven ( Group I ) predominantly unilateral disease was discovered by angiography ( renal-artery stenosis in six and hydronephrosis in one ) ; in the remaining seven ( Group II ) no rennal-artery abnormality was found .
	manualset3
88758	4	399675	5	NULL	NULL	0	NULL	renal-artery stenosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In seven ( Group I ) predominantly unilateral disease was discovered by angiography ( renal-artery stenosis in six and hydronephrosis in one ) ; in the remaining seven ( Group II ) no rennal-artery abnormality was found .
	manualset3
88759	5	399675	5	NULL	NULL	0	NULL	hydronephrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In seven ( Group I ) predominantly unilateral disease was discovered by angiography ( renal-artery stenosis in six and hydronephrosis in one ) ; in the remaining seven ( Group II ) no rennal-artery abnormality was found .
	manualset3
88760	6	399675	5	NULL	NULL	0	NULL	seven ( Group II ) 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In seven ( Group I ) predominantly unilateral disease was discovered by angiography ( renal-artery stenosis in six and hydronephrosis in one ) ; in the remaining seven ( Group II ) no rennal-artery abnormality was found .
	manualset3
88761	7	399675	5	NULL	NULL	0	NULL	rennal-artery abnormality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In seven ( Group I ) predominantly unilateral disease was discovered by angiography ( renal-artery stenosis in six and hydronephrosis in one ) ; in the remaining seven ( Group II ) no rennal-artery abnormality was found .
	manualset3
88762	1	399676	5	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Treatment of acute lymphoblastic leukemia in adults using higher doses of cytostatic agents ) .
	manualset3
88763	2	399676	5	NULL	NULL	0	NULL	acute lymphoblastic leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Treatment of acute lymphoblastic leukemia in adults using higher doses of cytostatic agents ) .
	manualset3
88764	3	399676	5	NULL	NULL	0	NULL	adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Treatment of acute lymphoblastic leukemia in adults using higher doses of cytostatic agents ) .
	manualset3
88765	4	399676	5	NULL	NULL	0	NULL	higher doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Treatment of acute lymphoblastic leukemia in adults using higher doses of cytostatic agents ) .
	manualset3
88766	5	399676	5	NULL	NULL	0	NULL	cytostatic agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Treatment of acute lymphoblastic leukemia in adults using higher doses of cytostatic agents ) .
	manualset3
88767	1	399677	5	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In short , this study showed that syndromes of HQD and HYD both displayed disturbed function of the vegetative nervous system , and their types and severities were correlated with the difference of Syndromes .
	manualset3
88768	2	399677	5	NULL	NULL	NULL	NULL	syndrome of HQD	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In short , this study showed that syndromes of HQD and HYD both displayed disturbed function of the vegetative nervous system , and their types and severities were correlated with the difference of Syndromes .
	manualset3
88769	3	399677	5	NULL	NULL	0	NULL	disturbed function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In short , this study showed that syndromes of HQD and HYD both displayed disturbed function of the vegetative nervous system , and their types and severities were correlated with the difference of Syndromes .
	manualset3
88770	4	399677	5	NULL	NULL	NULL	NULL	vegetative nervous system	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In short , this study showed that syndromes of HQD and HYD both displayed disturbed function of the vegetative nervous system , and their types and severities were correlated with the difference of Syndromes .
	manualset3
88771	5	399677	5	NULL	NULL	0	NULL	types	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In short , this study showed that syndromes of HQD and HYD both displayed disturbed function of the vegetative nervous system , and their types and severities were correlated with the difference of Syndromes .
	manualset3
88772	6	399677	5	NULL	NULL	0	NULL	severities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In short , this study showed that syndromes of HQD and HYD both displayed disturbed function of the vegetative nervous system , and their types and severities were correlated with the difference of Syndromes .
	manualset3
88773	7	399677	5	NULL	NULL	0	NULL	difference of Syndromes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In short , this study showed that syndromes of HQD and HYD both displayed disturbed function of the vegetative nervous system , and their types and severities were correlated with the difference of Syndromes .
	manualset3
91211	8	399677	5	NULL	NULL	0	NULL	syndrome of HYD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In short , this study showed that syndromes of HQD and HYD both displayed disturbed function of the vegetative nervous system , and their types and severities were correlated with the difference of Syndromes .
	manualset3
88774	1	399678	5	NULL	NULL	0	NULL	smokers ( n = 16 )	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In smokers ( n = 16 ) , the number of exfoliated cervicovaginal epithelial cells and leukocyte ascorbic acid levels was significantly higher ( p less than 0.01 , p less than 0.05 , respectively ) compared with nonsmokers ( n = 30 ) .
	manualset3
88775	2	399678	5	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In smokers ( n = 16 ) , the number of exfoliated cervicovaginal epithelial cells and leukocyte ascorbic acid levels was significantly higher ( p less than 0.01 , p less than 0.05 , respectively ) compared with nonsmokers ( n = 30 ) .
	manualset3
88776	3	399678	5	NULL	NULL	0	NULL	exfoliated cervicovaginal epithelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In smokers ( n = 16 ) , the number of exfoliated cervicovaginal epithelial cells and leukocyte ascorbic acid levels was significantly higher ( p less than 0.01 , p less than 0.05 , respectively ) compared with nonsmokers ( n = 30 ) .
	manualset3
88777	4	399678	5	NULL	NULL	0	NULL	leukocyte ascorbic acid levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In smokers ( n = 16 ) , the number of exfoliated cervicovaginal epithelial cells and leukocyte ascorbic acid levels was significantly higher ( p less than 0.01 , p less than 0.05 , respectively ) compared with nonsmokers ( n = 30 ) .
	manualset3
88778	5	399678	5	NULL	NULL	0	NULL	p less than 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In smokers ( n = 16 ) , the number of exfoliated cervicovaginal epithelial cells and leukocyte ascorbic acid levels was significantly higher ( p less than 0.01 , p less than 0.05 , respectively ) compared with nonsmokers ( n = 30 ) .
	manualset3
88779	6	399678	5	NULL	NULL	0	NULL	p less than 0.05	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In smokers ( n = 16 ) , the number of exfoliated cervicovaginal epithelial cells and leukocyte ascorbic acid levels was significantly higher ( p less than 0.01 , p less than 0.05 , respectively ) compared with nonsmokers ( n = 30 ) .
	manualset3
88780	7	399678	5	NULL	NULL	0	NULL	nonsmokers ( n = 30 )	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In smokers ( n = 16 ) , the number of exfoliated cervicovaginal epithelial cells and leukocyte ascorbic acid levels was significantly higher ( p less than 0.01 , p less than 0.05 , respectively ) compared with nonsmokers ( n = 30 ) .
	manualset3
88781	1	399679	5	NULL	NULL	0	NULL	smokers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In smokers , sex influences the relationship between emphysema and clinical features .
	manualset3
88782	2	399679	5	NULL	NULL	NULL	NULL	sex	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In smokers , sex influences the relationship between emphysema and clinical features .
	manualset3
88783	3	399679	5	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In smokers , sex influences the relationship between emphysema and clinical features .
	manualset3
88786	4	399679	5	NULL	NULL	0	NULL	emphysema	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In smokers , sex influences the relationship between emphysema and clinical features .
	manualset3
88787	5	399679	5	NULL	NULL	0	NULL	clinical features	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In smokers , sex influences the relationship between emphysema and clinical features .
	manualset3
88789	1	399680	5	NULL	NULL	0	NULL	fermentation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In subsequent , fermentation with hydrolysate , maximal ethanol yield was attained after 24h with 0.368 % of sulfuric acid .
	manualset3
88790	2	399680	5	NULL	NULL	0	NULL	hydrolysate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In subsequent , fermentation with hydrolysate , maximal ethanol yield was attained after 24h with 0.368 % of sulfuric acid .
	manualset3
88791	3	399680	5	NULL	NULL	0	NULL	maximal ethanol yield	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In subsequent , fermentation with hydrolysate , maximal ethanol yield was attained after 24h with 0.368 % of sulfuric acid .
	manualset3
88792	4	399680	5	NULL	NULL	0	NULL	 after 24h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In subsequent , fermentation with hydrolysate , maximal ethanol yield was attained after 24h with 0.368 % of sulfuric acid .
	manualset3
88793	5	399680	5	NULL	NULL	0	NULL	0.368 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In subsequent , fermentation with hydrolysate , maximal ethanol yield was attained after 24h with 0.368 % of sulfuric acid .
	manualset3
88794	6	399680	5	NULL	NULL	0	NULL	sulfuric acid	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In subsequent , fermentation with hydrolysate , maximal ethanol yield was attained after 24h with 0.368 % of sulfuric acid .
	manualset3
88798	1	399681	5	NULL	NULL	NULL	NULL	review	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In sum , this review suggests that QSOX enzymes play a significant role in oxidative folding of a large variety of proteins in a wide range of multicellular organisms .
	manualset3
88799	2	399681	5	NULL	NULL	NULL	NULL	QSOX enzymes	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In sum , this review suggests that QSOX enzymes play a significant role in oxidative folding of a large variety of proteins in a wide range of multicellular organisms .
	manualset3
88801	3	399681	5	NULL	NULL	NULL	NULL	significant role	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In sum , this review suggests that QSOX enzymes play a significant role in oxidative folding of a large variety of proteins in a wide range of multicellular organisms .
	manualset3
88802	4	399681	5	NULL	NULL	NULL	NULL	oxidative folding of a large variety of proteins	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In sum , this review suggests that QSOX enzymes play a significant role in oxidative folding of a large variety of proteins in a wide range of multicellular organisms .
	manualset3
88803	5	399681	5	NULL	NULL	NULL	NULL	wide range	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In sum , this review suggests that QSOX enzymes play a significant role in oxidative folding of a large variety of proteins in a wide range of multicellular organisms .
	manualset3
88804	6	399681	5	NULL	NULL	NULL	NULL	multicellular organisms	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In sum , this review suggests that QSOX enzymes play a significant role in oxidative folding of a large variety of proteins in a wide range of multicellular organisms .
	manualset3
88806	1	399682	5	NULL	NULL	0	NULL	140 positive smears	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , 140 positive smears were detected : 57 cases showed changes due to HPV , 63 LSIL , 15 HSIL , and 5 carcinomas .
	manualset3
88807	2	399682	5	NULL	NULL	0	NULL	57 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , 140 positive smears were detected : 57 cases showed changes due to HPV , 63 LSIL , 15 HSIL , and 5 carcinomas .
	manualset3
88808	3	399682	5	NULL	NULL	0	NULL	HPV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , 140 positive smears were detected : 57 cases showed changes due to HPV , 63 LSIL , 15 HSIL , and 5 carcinomas .
	manualset3
88809	4	399682	5	NULL	NULL	0	NULL	63 LSIL	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , 140 positive smears were detected : 57 cases showed changes due to HPV , 63 LSIL , 15 HSIL , and 5 carcinomas .
	manualset3
88810	5	399682	5	NULL	NULL	0	NULL	15 HSIL	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , 140 positive smears were detected : 57 cases showed changes due to HPV , 63 LSIL , 15 HSIL , and 5 carcinomas .
	manualset3
88811	6	399682	5	NULL	NULL	0	NULL	5 carcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , 140 positive smears were detected : 57 cases showed changes due to HPV , 63 LSIL , 15 HSIL , and 5 carcinomas .
	manualset3
88812	1	399683	5	NULL	NULL	0	NULL	cold-storage preservation with UW	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , cold-storage preservation with UW reduced endothelium-independent vascular relaxation by mechanisms other than competition with NO ; this requires further evaluation .
	manualset3
88813	2	399683	5	NULL	NULL	0	NULL	endothelium-independent vascular relaxation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , cold-storage preservation with UW reduced endothelium-independent vascular relaxation by mechanisms other than competition with NO ; this requires further evaluation .
	manualset3
88814	3	399683	5	NULL	NULL	0	NULL	mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , cold-storage preservation with UW reduced endothelium-independent vascular relaxation by mechanisms other than competition with NO ; this requires further evaluation .
	manualset3
88815	4	399683	5	NULL	NULL	0	NULL	competition with NO	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , cold-storage preservation with UW reduced endothelium-independent vascular relaxation by mechanisms other than competition with NO ; this requires further evaluation .
	manualset3
88816	5	399683	5	NULL	NULL	0	NULL	evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , cold-storage preservation with UW reduced endothelium-independent vascular relaxation by mechanisms other than competition with NO ; this requires further evaluation .
	manualset3
88817	1	399684	5	NULL	NULL	0	NULL	distinct expression patterns	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , distinct expression patterns were shown for PKC isoenzymes alpha , beta I , beta II , delta , and epsilon in the mouse kidney .
	manualset3
88818	2	399684	5	NULL	NULL	NULL	NULL	PKC isoenzyme alpha	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In summary , distinct expression patterns were shown for PKC isoenzymes alpha , beta I , beta II , delta , and epsilon in the mouse kidney .
	manualset3
88819	3	399684	5	NULL	NULL	NULL	NULL	PKC isoenzyme beta I	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In summary , distinct expression patterns were shown for PKC isoenzymes alpha , beta I , beta II , delta , and epsilon in the mouse kidney .
	manualset3
88820	4	399684	5	NULL	NULL	NULL	NULL	PKC isoenzyme beta II	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In summary , distinct expression patterns were shown for PKC isoenzymes alpha , beta I , beta II , delta , and epsilon in the mouse kidney .
	manualset3
88821	5	399684	5	NULL	NULL	0	NULL	PKC isoenzyme delta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , distinct expression patterns were shown for PKC isoenzymes alpha , beta I , beta II , delta , and epsilon in the mouse kidney .
	manualset3
88822	6	399684	5	NULL	NULL	0	NULL	PKC isoenzyme epsilon	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , distinct expression patterns were shown for PKC isoenzymes alpha , beta I , beta II , delta , and epsilon in the mouse kidney .
	manualset3
88823	7	399684	5	NULL	NULL	0	NULL	mouse kidney	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , distinct expression patterns were shown for PKC isoenzymes alpha , beta I , beta II , delta , and epsilon in the mouse kidney .
	manualset3
88824	1	399685	5	NULL	NULL	0	NULL	hepatic lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , most hepatic lesions can be correctly characterized by supplemental use of enhanced sonography ; practitioners should nevertheless be aware of atypical phenomena to be able to critically evaluate the findings .
	manualset3
88825	2	399685	5	NULL	NULL	NULL	NULL	supplemental use of enhanced sonography	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In summary , most hepatic lesions can be correctly characterized by supplemental use of enhanced sonography ; practitioners should nevertheless be aware of atypical phenomena to be able to critically evaluate the findings .
	manualset3
88826	3	399685	5	NULL	NULL	NULL	NULL	practitioners	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In summary , most hepatic lesions can be correctly characterized by supplemental use of enhanced sonography ; practitioners should nevertheless be aware of atypical phenomena to be able to critically evaluate the findings .
	manualset3
88827	4	399685	5	NULL	NULL	0	NULL	atypical phenomena	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , most hepatic lesions can be correctly characterized by supplemental use of enhanced sonography ; practitioners should nevertheless be aware of atypical phenomena to be able to critically evaluate the findings .
	manualset3
88828	5	399685	5	NULL	NULL	0	NULL	critically evaluate the findings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , most hepatic lesions can be correctly characterized by supplemental use of enhanced sonography ; practitioners should nevertheless be aware of atypical phenomena to be able to critically evaluate the findings .
	manualset3
88829	1	399686	5	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , our results suggest that the UL78 protein of HCMV traffics between the cell surface and cytoplasm , from where it might be recycled via early endosomes .
	manualset3
88830	2	399686	5	NULL	NULL	0	NULL	UL78 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , our results suggest that the UL78 protein of HCMV traffics between the cell surface and cytoplasm , from where it might be recycled via early endosomes .
	manualset3
88831	3	399686	5	NULL	NULL	0	NULL	HCMV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , our results suggest that the UL78 protein of HCMV traffics between the cell surface and cytoplasm , from where it might be recycled via early endosomes .
	manualset3
88832	4	399686	5	NULL	NULL	0	NULL	cell surface	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , our results suggest that the UL78 protein of HCMV traffics between the cell surface and cytoplasm , from where it might be recycled via early endosomes .
	manualset3
88833	5	399686	5	NULL	NULL	0	NULL	cytoplasm	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , our results suggest that the UL78 protein of HCMV traffics between the cell surface and cytoplasm , from where it might be recycled via early endosomes .
	manualset3
88834	6	399686	5	NULL	NULL	0	NULL	early endosomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , our results suggest that the UL78 protein of HCMV traffics between the cell surface and cytoplasm , from where it might be recycled via early endosomes .
	manualset3
88835	1	399687	5	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , our study shows that 5-HT is a potent regulator of human dendritic cell function , and that targeting serotoninergic receptors might be a promising approach for the treatment of inflammatory disorders .
	manualset3
88836	2	399687	5	NULL	NULL	0	NULL	5-HT	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , our study shows that 5-HT is a potent regulator of human dendritic cell function , and that targeting serotoninergic receptors might be a promising approach for the treatment of inflammatory disorders .
	manualset3
88839	3	399687	5	NULL	NULL	0	NULL	potent regulator	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , our study shows that 5-HT is a potent regulator of human dendritic cell function , and that targeting serotoninergic receptors might be a promising approach for the treatment of inflammatory disorders .
	manualset3
88840	4	399687	5	NULL	NULL	0	NULL	human dendritic cell function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , our study shows that 5-HT is a potent regulator of human dendritic cell function , and that targeting serotoninergic receptors might be a promising approach for the treatment of inflammatory disorders .
	manualset3
88841	5	399687	5	NULL	NULL	0	NULL	serotoninergic receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , our study shows that 5-HT is a potent regulator of human dendritic cell function , and that targeting serotoninergic receptors might be a promising approach for the treatment of inflammatory disorders .
	manualset3
88842	6	399687	5	NULL	NULL	0	NULL	promising approach	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , our study shows that 5-HT is a potent regulator of human dendritic cell function , and that targeting serotoninergic receptors might be a promising approach for the treatment of inflammatory disorders .
	manualset3
88843	7	399687	5	NULL	NULL	0	NULL	treatment of inflammatory disorders	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , our study shows that 5-HT is a potent regulator of human dendritic cell function , and that targeting serotoninergic receptors might be a promising approach for the treatment of inflammatory disorders .
	manualset3
88844	1	399688	5	NULL	NULL	0	NULL	 second and third trimester pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , second and third trimester pregnancy is associated with a normal circadian TSH rhythm .
	manualset3
88845	2	399688	5	NULL	NULL	0	NULL	normal circadian TSH rhythm	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , second and third trimester pregnancy is associated with a normal circadian TSH rhythm .
	manualset3
88848	1	399689	5	NULL	NULL	0	NULL	supplemental i.v. crystalloids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , supplemental i.v. crystalloids were associated with a lower incidence of several PONV outcomes .
	manualset3
88851	2	399689	5	NULL	NULL	0	NULL	lower incidence of several PONV outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , supplemental i.v. crystalloids were associated with a lower incidence of several PONV outcomes .
	manualset3
88853	1	399690	5	NULL	NULL	0	NULL	GICA TP-IgM	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , the characteristics of GICA TP-IgM correspond to that of FTA-Abs TP-IgM ; this can be used as a serologic marker for the relapse and infection of syphilis in place of the conventional FTA-Abs IgM test .
	manualset3
88854	2	399690	5	NULL	NULL	0	NULL	FTA-Abs TP-IgM	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , the characteristics of GICA TP-IgM correspond to that of FTA-Abs TP-IgM ; this can be used as a serologic marker for the relapse and infection of syphilis in place of the conventional FTA-Abs IgM test .
	manualset3
88855	3	399690	5	NULL	NULL	0	NULL	serologic marker	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , the characteristics of GICA TP-IgM correspond to that of FTA-Abs TP-IgM ; this can be used as a serologic marker for the relapse and infection of syphilis in place of the conventional FTA-Abs IgM test .
	manualset3
88857	4	399690	5	NULL	NULL	0	NULL	relapse and infection of syphilis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , the characteristics of GICA TP-IgM correspond to that of FTA-Abs TP-IgM ; this can be used as a serologic marker for the relapse and infection of syphilis in place of the conventional FTA-Abs IgM test .
	manualset3
88858	5	399690	5	NULL	NULL	0	NULL	conventional FTA-Abs IgM test 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , the characteristics of GICA TP-IgM correspond to that of FTA-Abs TP-IgM ; this can be used as a serologic marker for the relapse and infection of syphilis in place of the conventional FTA-Abs IgM test .
	manualset3
88859	1	399691	5	NULL	NULL	0	NULL	loss of 84 % of bulbospinal adrenergic neurones	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , the loss of 84 % of bulbospinal adrenergic neurones does not alter the ability of RVLM to maintain SNA and arterial pressure at rest in anaesthetized rats , but this loss reduces the sympathoexcitatory and pressor responses evoked by RVLM stimulation .
	manualset3
88860	2	399691	5	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , the loss of 84 % of bulbospinal adrenergic neurones does not alter the ability of RVLM to maintain SNA and arterial pressure at rest in anaesthetized rats , but this loss reduces the sympathoexcitatory and pressor responses evoked by RVLM stimulation .
	manualset3
88869	3	399691	5	NULL	NULL	0	NULL	RVLM	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , the loss of 84 % of bulbospinal adrenergic neurones does not alter the ability of RVLM to maintain SNA and arterial pressure at rest in anaesthetized rats , but this loss reduces the sympathoexcitatory and pressor responses evoked by RVLM stimulation .
	manualset3
88870	4	399691	5	NULL	NULL	0	NULL	SNA	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , the loss of 84 % of bulbospinal adrenergic neurones does not alter the ability of RVLM to maintain SNA and arterial pressure at rest in anaesthetized rats , but this loss reduces the sympathoexcitatory and pressor responses evoked by RVLM stimulation .
	manualset3
88871	5	399691	5	NULL	NULL	0	NULL	arterial pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , the loss of 84 % of bulbospinal adrenergic neurones does not alter the ability of RVLM to maintain SNA and arterial pressure at rest in anaesthetized rats , but this loss reduces the sympathoexcitatory and pressor responses evoked by RVLM stimulation .
	manualset3
88874	6	399691	5	NULL	NULL	0	NULL	anaesthetized rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , the loss of 84 % of bulbospinal adrenergic neurones does not alter the ability of RVLM to maintain SNA and arterial pressure at rest in anaesthetized rats , but this loss reduces the sympathoexcitatory and pressor responses evoked by RVLM stimulation .
	manualset3
88877	7	399691	5	NULL	NULL	0	NULL	sympathoexcitatory and pressor responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , the loss of 84 % of bulbospinal adrenergic neurones does not alter the ability of RVLM to maintain SNA and arterial pressure at rest in anaesthetized rats , but this loss reduces the sympathoexcitatory and pressor responses evoked by RVLM stimulation .
	manualset3
88878	8	399691	5	NULL	NULL	0	NULL	RVLM stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , the loss of 84 % of bulbospinal adrenergic neurones does not alter the ability of RVLM to maintain SNA and arterial pressure at rest in anaesthetized rats , but this loss reduces the sympathoexcitatory and pressor responses evoked by RVLM stimulation .
	manualset3
88879	1	399692	5	NULL	NULL	0	NULL	prevalence and incidence of upper urinary tract calculi	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , the prevalence and incidence of upper urinary tract calculi in the Tajima area were considerably higher than those in the nationwide survey on urolithiasis in Japan conducted in 1985 .
	manualset3
88880	2	399692	5	NULL	NULL	0	NULL	Tajima area	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , the prevalence and incidence of upper urinary tract calculi in the Tajima area were considerably higher than those in the nationwide survey on urolithiasis in Japan conducted in 1985 .
	manualset3
88886	3	399692	5	NULL	NULL	0	NULL	nationwide survey	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , the prevalence and incidence of upper urinary tract calculi in the Tajima area were considerably higher than those in the nationwide survey on urolithiasis in Japan conducted in 1985 .
	manualset3
88887	4	399692	5	NULL	NULL	0	NULL	urolithiasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , the prevalence and incidence of upper urinary tract calculi in the Tajima area were considerably higher than those in the nationwide survey on urolithiasis in Japan conducted in 1985 .
	manualset3
88888	5	399692	5	NULL	NULL	0	NULL	Japan	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , the prevalence and incidence of upper urinary tract calculi in the Tajima area were considerably higher than those in the nationwide survey on urolithiasis in Japan conducted in 1985 .
	manualset3
88889	6	399692	5	NULL	NULL	0	NULL	1985	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , the prevalence and incidence of upper urinary tract calculi in the Tajima area were considerably higher than those in the nationwide survey on urolithiasis in Japan conducted in 1985 .
	manualset3
88890	1	399693	5	NULL	NULL	0	NULL	testis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In testis , IMP1 and IMP3 were found mainly in the spermatogonia , whereas IMP2 was expressed in the immature Leydig cells .
	manualset3
88891	2	399693	5	NULL	NULL	0	NULL	IMP1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In testis , IMP1 and IMP3 were found mainly in the spermatogonia , whereas IMP2 was expressed in the immature Leydig cells .
	manualset3
88892	3	399693	5	NULL	NULL	0	NULL	IMP3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In testis , IMP1 and IMP3 were found mainly in the spermatogonia , whereas IMP2 was expressed in the immature Leydig cells .
	manualset3
88893	4	399693	5	NULL	NULL	0	NULL	spermatogonia	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In testis , IMP1 and IMP3 were found mainly in the spermatogonia , whereas IMP2 was expressed in the immature Leydig cells .
	manualset3
88894	5	399693	5	NULL	NULL	0	NULL	IMP2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In testis , IMP1 and IMP3 were found mainly in the spermatogonia , whereas IMP2 was expressed in the immature Leydig cells .
	manualset3
88895	6	399693	5	NULL	NULL	0	NULL	immature Leydig cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In testis , IMP1 and IMP3 were found mainly in the spermatogonia , whereas IMP2 was expressed in the immature Leydig cells .
	manualset3
88896	1	399694	5	NULL	NULL	0	NULL	Treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Treatment of hemorrhoids in pregnancy & puerperium ) .
	manualset3
88897	2	399694	5	NULL	NULL	NULL	NULL	hemorrhoids	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Treatment of hemorrhoids in pregnancy & puerperium ) .
	manualset3
88898	3	399694	5	NULL	NULL	NULL	NULL	pregnancy	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Treatment of hemorrhoids in pregnancy & puerperium ) .
	manualset3
88899	4	399694	5	NULL	NULL	NULL	NULL	puerperium	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Treatment of hemorrhoids in pregnancy & puerperium ) .
	manualset3
88936	1	399695	5	NULL	NULL	0	NULL	toddlers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In toddlers , iron requirements can be satisfied with a daily consumption of at least one serving of iron-containing foods , along with enhancers of iron absorption .
	manualset3
88937	2	399695	5	NULL	NULL	0	NULL	iron requirements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In toddlers , iron requirements can be satisfied with a daily consumption of at least one serving of iron-containing foods , along with enhancers of iron absorption .
	manualset3
88938	3	399695	5	NULL	NULL	0	NULL	daily consumption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In toddlers , iron requirements can be satisfied with a daily consumption of at least one serving of iron-containing foods , along with enhancers of iron absorption .
	manualset3
88939	4	399695	5	NULL	NULL	0	NULL	one serving of iron-containing foods	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	In toddlers , iron requirements can be satisfied with a daily consumption of at least one serving of iron-containing foods , along with enhancers of iron absorption .
	manualset3
88940	5	399695	5	NULL	NULL	0	NULL	enhancers of iron absorption	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In toddlers , iron requirements can be satisfied with a daily consumption of at least one serving of iron-containing foods , along with enhancers of iron absorption .
	manualset3
88979	1	399696	5	NULL	NULL	0	NULL	total	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In total , 81 patients with CDAD were reported ; 49 ( 61 % ) patients had nosocomial CDAD , and 29 ( 36 % ) patients were admitted to hospital when already suffering from diarrhoea .
	manualset3
88980	2	399696	5	NULL	NULL	0	NULL	81 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In total , 81 patients with CDAD were reported ; 49 ( 61 % ) patients had nosocomial CDAD , and 29 ( 36 % ) patients were admitted to hospital when already suffering from diarrhoea .
	manualset3
88981	3	399696	5	NULL	NULL	0	NULL	CDAD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In total , 81 patients with CDAD were reported ; 49 ( 61 % ) patients had nosocomial CDAD , and 29 ( 36 % ) patients were admitted to hospital when already suffering from diarrhoea .
	manualset3
88982	4	399696	5	NULL	NULL	0	NULL	49 ( 61 % ) patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In total , 81 patients with CDAD were reported ; 49 ( 61 % ) patients had nosocomial CDAD , and 29 ( 36 % ) patients were admitted to hospital when already suffering from diarrhoea .
	manualset3
88983	5	399696	5	NULL	NULL	0	NULL	nosocomial CDAD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In total , 81 patients with CDAD were reported ; 49 ( 61 % ) patients had nosocomial CDAD , and 29 ( 36 % ) patients were admitted to hospital when already suffering from diarrhoea .
	manualset3
88984	6	399696	5	NULL	NULL	0	NULL	29 ( 36 % ) patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In total , 81 patients with CDAD were reported ; 49 ( 61 % ) patients had nosocomial CDAD , and 29 ( 36 % ) patients were admitted to hospital when already suffering from diarrhoea .
	manualset3
88985	7	399696	5	NULL	NULL	0	NULL	hospital	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In total , 81 patients with CDAD were reported ; 49 ( 61 % ) patients had nosocomial CDAD , and 29 ( 36 % ) patients were admitted to hospital when already suffering from diarrhoea .
	manualset3
88986	8	399696	5	NULL	NULL	0	NULL	diarrhoea	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In total , 81 patients with CDAD were reported ; 49 ( 61 % ) patients had nosocomial CDAD , and 29 ( 36 % ) patients were admitted to hospital when already suffering from diarrhoea .
	manualset3
88988	2	399697	5	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In total , these results suggest that the use of chromatic information as a segmentation cue for motion integration relies on higher-level mechanisms , whereas luminance information works mainly through low-level motion mechanisms .
	manualset3
88989	3	399697	5	NULL	NULL	0	NULL	use of chromatic information	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In total , these results suggest that the use of chromatic information as a segmentation cue for motion integration relies on higher-level mechanisms , whereas luminance information works mainly through low-level motion mechanisms .
	manualset3
88990	4	399697	5	NULL	NULL	0	NULL	segmentation cue	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In total , these results suggest that the use of chromatic information as a segmentation cue for motion integration relies on higher-level mechanisms , whereas luminance information works mainly through low-level motion mechanisms .
	manualset3
88991	5	399697	5	NULL	NULL	0	NULL	motion integration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In total , these results suggest that the use of chromatic information as a segmentation cue for motion integration relies on higher-level mechanisms , whereas luminance information works mainly through low-level motion mechanisms .
	manualset3
88992	6	399697	5	NULL	NULL	0	NULL	higher-level mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In total , these results suggest that the use of chromatic information as a segmentation cue for motion integration relies on higher-level mechanisms , whereas luminance information works mainly through low-level motion mechanisms .
	manualset3
88993	7	399697	5	NULL	NULL	0	NULL	luminance information	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In total , these results suggest that the use of chromatic information as a segmentation cue for motion integration relies on higher-level mechanisms , whereas luminance information works mainly through low-level motion mechanisms .
	manualset3
88994	8	399697	5	NULL	NULL	0	NULL	low-level motion mechanisms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In total , these results suggest that the use of chromatic information as a segmentation cue for motion integration relies on higher-level mechanisms , whereas luminance information works mainly through low-level motion mechanisms .
	manualset3
88995	1	399698	5	NULL	NULL	0	NULL	transcription	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In transcription , an unnatural base pair system could be used for making new RNA molecules containing functional components of interest at specific positions .
	manualset3
88996	2	399698	5	NULL	NULL	0	NULL	unnatural base pair system	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In transcription , an unnatural base pair system could be used for making new RNA molecules containing functional components of interest at specific positions .
	manualset3
88997	3	399698	5	NULL	NULL	0	NULL	new RNA molecules	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In transcription , an unnatural base pair system could be used for making new RNA molecules containing functional components of interest at specific positions .
	manualset3
88998	4	399698	5	NULL	NULL	0	NULL	 functional components of interest	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In transcription , an unnatural base pair system could be used for making new RNA molecules containing functional components of interest at specific positions .
	manualset3
88999	5	399698	5	NULL	NULL	0	NULL	specific positions	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In transcription , an unnatural base pair system could be used for making new RNA molecules containing functional components of interest at specific positions .
	manualset3
89000	1	399699	5	NULL	NULL	NULL	NULL	expression of high levels of neurotrophins	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In turn , there is expression of high levels of neurotrophins at the invasion front of normal tissue adjacent to brain metastases , thus implicating this growth factor-receptor system in melanoma tumorigenesis .
	manualset3
89001	2	399699	5	NULL	NULL	0	NULL	invasion front of normal tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In turn , there is expression of high levels of neurotrophins at the invasion front of normal tissue adjacent to brain metastases , thus implicating this growth factor-receptor system in melanoma tumorigenesis .
	manualset3
89002	3	399699	5	NULL	NULL	0	NULL	brain metastases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In turn , there is expression of high levels of neurotrophins at the invasion front of normal tissue adjacent to brain metastases , thus implicating this growth factor-receptor system in melanoma tumorigenesis .
	manualset3
89003	4	399699	5	NULL	NULL	NULL	NULL	growth factor-receptor system	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In turn , there is expression of high levels of neurotrophins at the invasion front of normal tissue adjacent to brain metastases , thus implicating this growth factor-receptor system in melanoma tumorigenesis .
	manualset3
89004	5	399699	5	NULL	NULL	0	NULL	melanoma tumorigenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In turn , there is expression of high levels of neurotrophins at the invasion front of normal tissue adjacent to brain metastases , thus implicating this growth factor-receptor system in melanoma tumorigenesis .
	manualset3
89005	1	399700	5	NULL	NULL	0	NULL	+ / - 70 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In + / - 70 % of all infants with congential infections relapses of chorioretinitis give rise to scars in their eyes after a follow-up of 16 years .
	manualset3
89006	2	399700	5	NULL	NULL	0	NULL	infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In + / - 70 % of all infants with congential infections relapses of chorioretinitis give rise to scars in their eyes after a follow-up of 16 years .
	manualset3
89007	3	399700	5	NULL	NULL	0	NULL	congential infections relapses of chorioretinitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In + / - 70 % of all infants with congential infections relapses of chorioretinitis give rise to scars in their eyes after a follow-up of 16 years .
	manualset3
89008	4	399700	5	NULL	NULL	0	NULL	scars	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In + / - 70 % of all infants with congential infections relapses of chorioretinitis give rise to scars in their eyes after a follow-up of 16 years .
	manualset3
89009	5	399700	5	NULL	NULL	0	NULL	eyes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In + / - 70 % of all infants with congential infections relapses of chorioretinitis give rise to scars in their eyes after a follow-up of 16 years .
	manualset3
89010	6	399700	5	NULL	NULL	0	NULL	 follow-up of 16 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In + / - 70 % of all infants with congential infections relapses of chorioretinitis give rise to scars in their eyes after a follow-up of 16 years .
	manualset3
89011	1	399701	5	NULL	NULL	0	NULL	1 patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1 patient , surgery had to be limited to removal of an intracerebral hematoma .
	manualset3
89012	2	399701	5	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1 patient , surgery had to be limited to removal of an intracerebral hematoma .
	manualset3
89013	3	399701	5	NULL	NULL	0	NULL	removal of an intracerebral hematoma	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1 patient , surgery had to be limited to removal of an intracerebral hematoma .
	manualset3
89014	1	399702	5	NULL	NULL	0	NULL	10 Wistar rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In 10 Wistar rats , the anatomy of the external jugular vein was studied by dissection and histology .
	manualset3
89015	2	399702	5	NULL	NULL	0	NULL	anatomy	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 10 Wistar rats , the anatomy of the external jugular vein was studied by dissection and histology .
	manualset3
89016	3	399702	5	NULL	NULL	0	NULL	external jugular vein	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In 10 Wistar rats , the anatomy of the external jugular vein was studied by dissection and histology .
	manualset3
89017	4	399702	5	NULL	NULL	0	NULL	dissection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 10 Wistar rats , the anatomy of the external jugular vein was studied by dissection and histology .
	manualset3
89018	5	399702	5	NULL	NULL	0	NULL	histology	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 10 Wistar rats , the anatomy of the external jugular vein was studied by dissection and histology .
	manualset3
89019	1	399703	5	NULL	NULL	0	NULL	Anthropometric criteria	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Anthropometric criteria in the diagnosis of malnutrition in child care programs ) .
	manualset3
89020	2	399703	5	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Anthropometric criteria in the diagnosis of malnutrition in child care programs ) .
	manualset3
89021	3	399703	5	NULL	NULL	0	NULL	malnutrition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Anthropometric criteria in the diagnosis of malnutrition in child care programs ) .
	manualset3
89022	4	399703	5	NULL	NULL	NULL	NULL	child care programs	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Anthropometric criteria in the diagnosis of malnutrition in child care programs ) .
	manualset3
89023	1	399704	5	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Treatment of hypercalcemia with mithramycin ) .
	manualset3
89024	2	399704	5	NULL	NULL	0	NULL	hypercalcemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Treatment of hypercalcemia with mithramycin ) .
	manualset3
89025	3	399704	5	NULL	NULL	0	NULL	mithramycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Treatment of hypercalcemia with mithramycin ) .
	manualset3
89026	1	399705	5	NULL	NULL	0	NULL	10	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In 10 of these subjects , transit of the tablet was delayed in the esophagus .
	manualset3
89027	2	399705	5	NULL	NULL	0	NULL	subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 10 of these subjects , transit of the tablet was delayed in the esophagus .
	manualset3
89029	3	399705	5	NULL	NULL	0	NULL	transit of the tablet	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In 10 of these subjects , transit of the tablet was delayed in the esophagus .
	manualset3
89030	4	399705	5	NULL	NULL	0	NULL	esophagus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In 10 of these subjects , transit of the tablet was delayed in the esophagus .
	manualset3
89031	1	399706	5	NULL	NULL	0	NULL	10 patients ( 77 % )	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 10 patients ( 77 % ) , vasospasm was due to subarachnoid hemorrhage following rupture of an intracranial aneurysm .
	manualset3
89033	2	399706	5	NULL	NULL	0	NULL	vasospasm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 10 patients ( 77 % ) , vasospasm was due to subarachnoid hemorrhage following rupture of an intracranial aneurysm .
	manualset3
89034	3	399706	5	NULL	NULL	0	NULL	subarachnoid hemorrhage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 10 patients ( 77 % ) , vasospasm was due to subarachnoid hemorrhage following rupture of an intracranial aneurysm .
	manualset3
89036	4	399706	5	NULL	NULL	0	NULL	rupture of an intracranial aneurysm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 10 patients ( 77 % ) , vasospasm was due to subarachnoid hemorrhage following rupture of an intracranial aneurysm .
	manualset3
89037	1	399707	5	NULL	NULL	0	NULL	10 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 10 patients treated by surgical excision and chemotherapy , serum gamma-enolase was significantly reduced after the treatment .
	manualset3
89038	2	399707	5	NULL	NULL	0	NULL	surgical excision	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 10 patients treated by surgical excision and chemotherapy , serum gamma-enolase was significantly reduced after the treatment .
	manualset3
89039	3	399707	5	NULL	NULL	0	NULL	chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 10 patients treated by surgical excision and chemotherapy , serum gamma-enolase was significantly reduced after the treatment .
	manualset3
89040	4	399707	5	NULL	NULL	0	NULL	serum gamma-enolase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In 10 patients treated by surgical excision and chemotherapy , serum gamma-enolase was significantly reduced after the treatment .
	manualset3
89041	5	399707	5	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 10 patients treated by surgical excision and chemotherapy , serum gamma-enolase was significantly reduced after the treatment .
	manualset3
89042	1	399708	5	NULL	NULL	0	NULL	10 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 10 patients with myasthenia gravis , we studied the relationship between plasma pyridostigmine levels and five measures of neuromuscular function ( NMF ) following single oral doses of 60 to 120 mg .
	manualset3
89043	2	399708	5	NULL	NULL	0	NULL	myasthenia gravis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In 10 patients with myasthenia gravis , we studied the relationship between plasma pyridostigmine levels and five measures of neuromuscular function ( NMF ) following single oral doses of 60 to 120 mg .
	manualset3
89044	3	399708	5	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In 10 patients with myasthenia gravis , we studied the relationship between plasma pyridostigmine levels and five measures of neuromuscular function ( NMF ) following single oral doses of 60 to 120 mg .
	manualset3
89045	4	399708	5	NULL	NULL	0	NULL	plasma pyridostigmine levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 10 patients with myasthenia gravis , we studied the relationship between plasma pyridostigmine levels and five measures of neuromuscular function ( NMF ) following single oral doses of 60 to 120 mg .
	manualset3
89046	5	399708	5	NULL	NULL	0	NULL	five measures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 10 patients with myasthenia gravis , we studied the relationship between plasma pyridostigmine levels and five measures of neuromuscular function ( NMF ) following single oral doses of 60 to 120 mg .
	manualset3
89047	6	399708	5	NULL	NULL	0	NULL	neuromuscular function ( NMF )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In 10 patients with myasthenia gravis , we studied the relationship between plasma pyridostigmine levels and five measures of neuromuscular function ( NMF ) following single oral doses of 60 to 120 mg .
	manualset3
89048	7	399708	5	NULL	NULL	0	NULL	single oral doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 10 patients with myasthenia gravis , we studied the relationship between plasma pyridostigmine levels and five measures of neuromuscular function ( NMF ) following single oral doses of 60 to 120 mg .
	manualset3
89051	8	399708	5	NULL	NULL	0	NULL	60 to 120 mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In 10 patients with myasthenia gravis , we studied the relationship between plasma pyridostigmine levels and five measures of neuromuscular function ( NMF ) following single oral doses of 60 to 120 mg .
	manualset3
89054	1	399709	5	NULL	NULL	0	NULL	100 evaluable patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 100 evaluable patients , the objective response rates were 35 % for VMP and 61 % for VAP , the complete response rates being 6 % and 13 % , respectively .
	manualset3
89059	2	399709	5	NULL	NULL	0	NULL	objective response rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 100 evaluable patients , the objective response rates were 35 % for VMP and 61 % for VAP , the complete response rates being 6 % and 13 % , respectively .
	manualset3
89060	3	399709	5	NULL	NULL	0	NULL	35 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In 100 evaluable patients , the objective response rates were 35 % for VMP and 61 % for VAP , the complete response rates being 6 % and 13 % , respectively .
	manualset3
89061	4	399709	5	NULL	NULL	0	NULL	VMP	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In 100 evaluable patients , the objective response rates were 35 % for VMP and 61 % for VAP , the complete response rates being 6 % and 13 % , respectively .
	manualset3
89062	5	399709	5	NULL	NULL	0	NULL	61 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In 100 evaluable patients , the objective response rates were 35 % for VMP and 61 % for VAP , the complete response rates being 6 % and 13 % , respectively .
	manualset3
89063	6	399709	5	NULL	NULL	0	NULL	VAP	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In 100 evaluable patients , the objective response rates were 35 % for VMP and 61 % for VAP , the complete response rates being 6 % and 13 % , respectively .
	manualset3
89064	7	399709	5	NULL	NULL	0	NULL	complete response rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 100 evaluable patients , the objective response rates were 35 % for VMP and 61 % for VAP , the complete response rates being 6 % and 13 % , respectively .
	manualset3
89065	8	399709	5	NULL	NULL	NULL	NULL	 6 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In 100 evaluable patients , the objective response rates were 35 % for VMP and 61 % for VAP , the complete response rates being 6 % and 13 % , respectively .
	manualset3
91212	9	399709	5	NULL	NULL	0	NULL	13 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In 100 evaluable patients , the objective response rates were 35 % for VMP and 61 % for VAP , the complete response rates being 6 % and 13 % , respectively .
	manualset3
89068	1	399710	5	NULL	NULL	0	NULL	105 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 105 patients injecting themselves insulin of the diabetes department of the municipal hospital Dresden-Neustadt with an average age of 63.3 years the HBs-antigen was determined for the purpose of testing the degree of contamination .
	manualset3
89075	2	399710	5	NULL	NULL	NULL	NULL	insulin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In 105 patients injecting themselves insulin of the diabetes department of the municipal hospital Dresden-Neustadt with an average age of 63.3 years the HBs-antigen was determined for the purpose of testing the degree of contamination .
	manualset3
89076	3	399710	5	NULL	NULL	0	NULL	diabetes department of the municipal hospital	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In 105 patients injecting themselves insulin of the diabetes department of the municipal hospital Dresden-Neustadt with an average age of 63.3 years the HBs-antigen was determined for the purpose of testing the degree of contamination .
	manualset3
89077	4	399710	5	NULL	NULL	0	NULL	Dresden-Neustadt 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In 105 patients injecting themselves insulin of the diabetes department of the municipal hospital Dresden-Neustadt with an average age of 63.3 years the HBs-antigen was determined for the purpose of testing the degree of contamination .
	manualset3
89080	5	399710	5	NULL	NULL	NULL	NULL	average age of 63.3 years	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In 105 patients injecting themselves insulin of the diabetes department of the municipal hospital Dresden-Neustadt with an average age of 63.3 years the HBs-antigen was determined for the purpose of testing the degree of contamination .
	manualset3
89084	6	399710	5	NULL	NULL	0	NULL	HBs-antigen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In 105 patients injecting themselves insulin of the diabetes department of the municipal hospital Dresden-Neustadt with an average age of 63.3 years the HBs-antigen was determined for the purpose of testing the degree of contamination .
	manualset3
89085	7	399710	5	NULL	NULL	0	NULL	degree of contamination	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 105 patients injecting themselves insulin of the diabetes department of the municipal hospital Dresden-Neustadt with an average age of 63.3 years the HBs-antigen was determined for the purpose of testing the degree of contamination .
	manualset3
89088	1	399711	5	NULL	NULL	0	NULL	121 patients ( 72 % )	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 121 patients ( 72 % ) therapeutic decision was based on IVU , ultrasound , and cytology alone .
	manualset3
89089	2	399711	5	NULL	NULL	NULL	NULL	therapeutic decision	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In 121 patients ( 72 % ) therapeutic decision was based on IVU , ultrasound , and cytology alone .
	manualset3
89094	3	399711	5	NULL	NULL	0	NULL	IVU	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 121 patients ( 72 % ) therapeutic decision was based on IVU , ultrasound , and cytology alone .
	manualset3
89096	4	399711	5	NULL	NULL	0	NULL	ultrasound	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 121 patients ( 72 % ) therapeutic decision was based on IVU , ultrasound , and cytology alone .
	manualset3
89099	5	399711	5	NULL	NULL	0	NULL	cytology	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 121 patients ( 72 % ) therapeutic decision was based on IVU , ultrasound , and cytology alone .
	manualset3
89101	1	399712	5	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Treatment of lipoid nephrosis in the child ) .
	manualset3
89102	2	399712	5	NULL	NULL	0	NULL	lipoid nephrosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Treatment of lipoid nephrosis in the child ) .
	manualset3
89103	3	399712	5	NULL	NULL	0	NULL	child	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( Treatment of lipoid nephrosis in the child ) .
	manualset3
89104	1	399713	5	NULL	NULL	0	NULL	13 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 13 cases the EEG was abnormal , the abnormality most frequently observed being a of the rhythmic slow wave type , consisting of bursts of monorhythmic theta or delta waves seen in both hemispheres .
	manualset3
89105	2	399713	5	NULL	NULL	0	NULL	EEG	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 13 cases the EEG was abnormal , the abnormality most frequently observed being a of the rhythmic slow wave type , consisting of bursts of monorhythmic theta or delta waves seen in both hemispheres .
	manualset3
89106	3	399713	5	NULL	NULL	0	NULL	abnormality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 13 cases the EEG was abnormal , the abnormality most frequently observed being a of the rhythmic slow wave type , consisting of bursts of monorhythmic theta or delta waves seen in both hemispheres .
	manualset3
89107	4	399713	5	NULL	NULL	0	NULL	 rhythmic slow wave type	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 13 cases the EEG was abnormal , the abnormality most frequently observed being a of the rhythmic slow wave type , consisting of bursts of monorhythmic theta or delta waves seen in both hemispheres .
	manualset3
89108	5	399713	5	NULL	NULL	NULL	NULL	bursts of monorhythmic theta or delta waves	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In 13 cases the EEG was abnormal , the abnormality most frequently observed being a of the rhythmic slow wave type , consisting of bursts of monorhythmic theta or delta waves seen in both hemispheres .
	manualset3
89109	6	399713	5	NULL	NULL	NULL	NULL	hemispheres	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In 13 cases the EEG was abnormal , the abnormality most frequently observed being a of the rhythmic slow wave type , consisting of bursts of monorhythmic theta or delta waves seen in both hemispheres .
	manualset3
89110	1	399714	5	NULL	NULL	0	NULL	15 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 15 cases the glucose tolerance curves were indicative of diabetes , in seven cases questionable and in ten cases normal .
	manualset3
89111	2	399714	5	NULL	NULL	NULL	NULL	glucose tolerance curves	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In 15 cases the glucose tolerance curves were indicative of diabetes , in seven cases questionable and in ten cases normal .
	manualset3
89112	3	399714	5	NULL	NULL	0	NULL	diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In 15 cases the glucose tolerance curves were indicative of diabetes , in seven cases questionable and in ten cases normal .
	manualset3
89113	4	399714	5	NULL	NULL	0	NULL	seven cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 15 cases the glucose tolerance curves were indicative of diabetes , in seven cases questionable and in ten cases normal .
	manualset3
89114	5	399714	5	NULL	NULL	0	NULL	ten cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 15 cases the glucose tolerance curves were indicative of diabetes , in seven cases questionable and in ten cases normal .
	manualset3
89115	6	399714	5	NULL	NULL	0	NULL	normal	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 15 cases the glucose tolerance curves were indicative of diabetes , in seven cases questionable and in ten cases normal .
	manualset3
89116	1	399715	5	NULL	NULL	0	NULL	15 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 15 patients with extrahepatic biliary obstruction , the average hepatocyte clearance was disproportionately increased , as in IC , but large-duct obstruction was identified by scintigrams , ultrasound , or computed tomography .
	manualset3
89117	2	399715	5	NULL	NULL	0	NULL	extrahepatic biliary obstruction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 15 patients with extrahepatic biliary obstruction , the average hepatocyte clearance was disproportionately increased , as in IC , but large-duct obstruction was identified by scintigrams , ultrasound , or computed tomography .
	manualset3
89118	3	399715	5	NULL	NULL	0	NULL	average hepatocyte clearance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In 15 patients with extrahepatic biliary obstruction , the average hepatocyte clearance was disproportionately increased , as in IC , but large-duct obstruction was identified by scintigrams , ultrasound , or computed tomography .
	manualset3
89119	4	399715	5	NULL	NULL	0	NULL	IC	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 15 patients with extrahepatic biliary obstruction , the average hepatocyte clearance was disproportionately increased , as in IC , but large-duct obstruction was identified by scintigrams , ultrasound , or computed tomography .
	manualset3
89120	5	399715	5	NULL	NULL	0	NULL	large-duct obstruction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 15 patients with extrahepatic biliary obstruction , the average hepatocyte clearance was disproportionately increased , as in IC , but large-duct obstruction was identified by scintigrams , ultrasound , or computed tomography .
	manualset3
89121	6	399715	5	NULL	NULL	NULL	NULL	scintigrams	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In 15 patients with extrahepatic biliary obstruction , the average hepatocyte clearance was disproportionately increased , as in IC , but large-duct obstruction was identified by scintigrams , ultrasound , or computed tomography .
	manualset3
89122	7	399715	5	NULL	NULL	0	NULL	ultrasound	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 15 patients with extrahepatic biliary obstruction , the average hepatocyte clearance was disproportionately increased , as in IC , but large-duct obstruction was identified by scintigrams , ultrasound , or computed tomography .
	manualset3
89123	8	399715	5	NULL	NULL	0	NULL	computed tomography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 15 patients with extrahepatic biliary obstruction , the average hepatocyte clearance was disproportionately increased , as in IC , but large-duct obstruction was identified by scintigrams , ultrasound , or computed tomography .
	manualset3
89124	1	399716	5	NULL	NULL	0	NULL	15 years ( 1964-1979 )	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In 15 years ( 1964-1979 ) 415 primary central nervous system tumors were studied and treated ; 67 corresponded to tumors with risk of meningeal dissemination .
	manualset3
89125	2	399716	5	NULL	NULL	0	NULL	415 primary central nervous system tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 15 years ( 1964-1979 ) 415 primary central nervous system tumors were studied and treated ; 67 corresponded to tumors with risk of meningeal dissemination .
	manualset3
89126	3	399716	5	NULL	NULL	0	NULL	67	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In 15 years ( 1964-1979 ) 415 primary central nervous system tumors were studied and treated ; 67 corresponded to tumors with risk of meningeal dissemination .
	manualset3
89127	4	399716	5	NULL	NULL	NULL	NULL	tumors with risk of meningeal dissemination	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In 15 years ( 1964-1979 ) 415 primary central nervous system tumors were studied and treated ; 67 corresponded to tumors with risk of meningeal dissemination .
	manualset3
89128	1	399717	5	NULL	NULL	0	NULL	17 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 17 patients planar anterior imaging of the heart was performed 5 min and 120 min p.i. During this time interval , mean decay-corrected myocardial activity declined to 77.9 % + / - 9.7 % after stress and to 85.7 % + / - 7.9 % after injection at rest ( P & lt ; 0.05 ) .
	manualset3
89129	2	399717	5	NULL	NULL	0	NULL	planar anterior imaging 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 17 patients planar anterior imaging of the heart was performed 5 min and 120 min p.i. During this time interval , mean decay-corrected myocardial activity declined to 77.9 % + / - 9.7 % after stress and to 85.7 % + / - 7.9 % after injection at rest ( P & lt ; 0.05 ) .
	manualset3
89130	3	399717	5	NULL	NULL	0	NULL	heart	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In 17 patients planar anterior imaging of the heart was performed 5 min and 120 min p.i. During this time interval , mean decay-corrected myocardial activity declined to 77.9 % + / - 9.7 % after stress and to 85.7 % + / - 7.9 % after injection at rest ( P & lt ; 0.05 ) .
	manualset3
89131	4	399717	5	NULL	NULL	0	NULL	5 min and 120 min	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	In 17 patients planar anterior imaging of the heart was performed 5 min and 120 min p.i. During this time interval , mean decay-corrected myocardial activity declined to 77.9 % + / - 9.7 % after stress and to 85.7 % + / - 7.9 % after injection at rest ( P & lt ; 0.05 ) .
	manualset3
89132	5	399717	5	NULL	NULL	0	NULL	time interval	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In 17 patients planar anterior imaging of the heart was performed 5 min and 120 min p.i. During this time interval , mean decay-corrected myocardial activity declined to 77.9 % + / - 9.7 % after stress and to 85.7 % + / - 7.9 % after injection at rest ( P & lt ; 0.05 ) .
	manualset3
89133	6	399717	5	NULL	NULL	0	NULL	mean decay-corrected myocardial activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In 17 patients planar anterior imaging of the heart was performed 5 min and 120 min p.i. During this time interval , mean decay-corrected myocardial activity declined to 77.9 % + / - 9.7 % after stress and to 85.7 % + / - 7.9 % after injection at rest ( P & lt ; 0.05 ) .
	manualset3
89134	7	399717	5	NULL	NULL	0	NULL	77.9 % + / - 9.7 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In 17 patients planar anterior imaging of the heart was performed 5 min and 120 min p.i. During this time interval , mean decay-corrected myocardial activity declined to 77.9 % + / - 9.7 % after stress and to 85.7 % + / - 7.9 % after injection at rest ( P & lt ; 0.05 ) .
	manualset3
89135	8	399717	5	NULL	NULL	0	NULL	stress	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In 17 patients planar anterior imaging of the heart was performed 5 min and 120 min p.i. During this time interval , mean decay-corrected myocardial activity declined to 77.9 % + / - 9.7 % after stress and to 85.7 % + / - 7.9 % after injection at rest ( P & lt ; 0.05 ) .
	manualset3
89136	9	399717	5	NULL	NULL	0	NULL	85.7 % + / - 7.9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In 17 patients planar anterior imaging of the heart was performed 5 min and 120 min p.i. During this time interval , mean decay-corrected myocardial activity declined to 77.9 % + / - 9.7 % after stress and to 85.7 % + / - 7.9 % after injection at rest ( P & lt ; 0.05 ) .
	manualset3
89137	10	399717	5	NULL	NULL	0	NULL	injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 17 patients planar anterior imaging of the heart was performed 5 min and 120 min p.i. During this time interval , mean decay-corrected myocardial activity declined to 77.9 % + / - 9.7 % after stress and to 85.7 % + / - 7.9 % after injection at rest ( P & lt ; 0.05 ) .
	manualset3
89138	11	399717	5	NULL	NULL	0	NULL	P & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In 17 patients planar anterior imaging of the heart was performed 5 min and 120 min p.i. During this time interval , mean decay-corrected myocardial activity declined to 77.9 % + / - 9.7 % after stress and to 85.7 % + / - 7.9 % after injection at rest ( P & lt ; 0.05 ) .
	manualset3
89139	1	399718	5	NULL	NULL	0	NULL	18 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 18 cases the fracture involved the proximal and in 16 cases the middle third of the scaphoid .
	manualset3
89140	2	399718	5	NULL	NULL	0	NULL	fracture	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 18 cases the fracture involved the proximal and in 16 cases the middle third of the scaphoid .
	manualset3
89141	3	399718	5	NULL	NULL	0	NULL	proximal	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In 18 cases the fracture involved the proximal and in 16 cases the middle third of the scaphoid .
	manualset3
89142	4	399718	5	NULL	NULL	0	NULL	16 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 18 cases the fracture involved the proximal and in 16 cases the middle third of the scaphoid .
	manualset3
89143	5	399718	5	NULL	NULL	0	NULL	middle third of the scaphoid	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In 18 cases the fracture involved the proximal and in 16 cases the middle third of the scaphoid .
	manualset3
89144	1	399719	5	NULL	NULL	0	NULL	18 specimens	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 18 specimens , the staining was fibrillar , was located in the upper half of the dermis , and was similar to the distribution of elastic fibers .
	manualset3
89145	2	399719	5	NULL	NULL	0	NULL	upper half of the dermis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In 18 specimens , the staining was fibrillar , was located in the upper half of the dermis , and was similar to the distribution of elastic fibers .
	manualset3
89146	3	399719	5	NULL	NULL	0	NULL	distribution of elastic fibers	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In 18 specimens , the staining was fibrillar , was located in the upper half of the dermis , and was similar to the distribution of elastic fibers .
	manualset3
89147	1	399720	5	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Treatment of varicose ulcers of the leg with xenogenic dura mater of the animal ) .
	manualset3
89148	2	399720	5	NULL	NULL	0	NULL	varicose ulcers	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Treatment of varicose ulcers of the leg with xenogenic dura mater of the animal ) .
	manualset3
89149	3	399720	5	NULL	NULL	0	NULL	leg	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Treatment of varicose ulcers of the leg with xenogenic dura mater of the animal ) .
	manualset3
89150	4	399720	5	NULL	NULL	0	NULL	xenogenic dura mater	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Treatment of varicose ulcers of the leg with xenogenic dura mater of the animal ) .
	manualset3
89151	5	399720	5	NULL	NULL	0	NULL	animal	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Treatment of varicose ulcers of the leg with xenogenic dura mater of the animal ) .
	manualset3
89152	1	399721	5	NULL	NULL	0	NULL	1932	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1932 Sherrington and Adrian were awarded the Nobel Prize in Physiology or Medicine `` for their discoveries regarding the functions of neurons '' and in 1944 Erlanger and Gasser were awarded the same prize `` for their discoveries relating to the highly differentiated functions of single nerve fibers . ''
	manualset3
89153	2	399721	5	NULL	NULL	0	NULL	Sherrington	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1932 Sherrington and Adrian were awarded the Nobel Prize in Physiology or Medicine `` for their discoveries regarding the functions of neurons '' and in 1944 Erlanger and Gasser were awarded the same prize `` for their discoveries relating to the highly differentiated functions of single nerve fibers . ''
	manualset3
89154	3	399721	5	NULL	NULL	0	NULL	Adrian	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1932 Sherrington and Adrian were awarded the Nobel Prize in Physiology or Medicine `` for their discoveries regarding the functions of neurons '' and in 1944 Erlanger and Gasser were awarded the same prize `` for their discoveries relating to the highly differentiated functions of single nerve fibers . ''
	manualset3
89155	4	399721	5	NULL	NULL	0	NULL	Nobel Prize in Physiology or Medicine	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1932 Sherrington and Adrian were awarded the Nobel Prize in Physiology or Medicine `` for their discoveries regarding the functions of neurons '' and in 1944 Erlanger and Gasser were awarded the same prize `` for their discoveries relating to the highly differentiated functions of single nerve fibers . ''
	manualset3
89156	5	399721	5	NULL	NULL	0	NULL	functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1932 Sherrington and Adrian were awarded the Nobel Prize in Physiology or Medicine `` for their discoveries regarding the functions of neurons '' and in 1944 Erlanger and Gasser were awarded the same prize `` for their discoveries relating to the highly differentiated functions of single nerve fibers . ''
	manualset3
89157	6	399721	5	NULL	NULL	0	NULL	neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1932 Sherrington and Adrian were awarded the Nobel Prize in Physiology or Medicine `` for their discoveries regarding the functions of neurons '' and in 1944 Erlanger and Gasser were awarded the same prize `` for their discoveries relating to the highly differentiated functions of single nerve fibers . ''
	manualset3
89158	7	399721	5	NULL	NULL	0	NULL	1944	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1932 Sherrington and Adrian were awarded the Nobel Prize in Physiology or Medicine `` for their discoveries regarding the functions of neurons '' and in 1944 Erlanger and Gasser were awarded the same prize `` for their discoveries relating to the highly differentiated functions of single nerve fibers . ''
	manualset3
89159	8	399721	5	NULL	NULL	0	NULL	Erlanger	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1932 Sherrington and Adrian were awarded the Nobel Prize in Physiology or Medicine `` for their discoveries regarding the functions of neurons '' and in 1944 Erlanger and Gasser were awarded the same prize `` for their discoveries relating to the highly differentiated functions of single nerve fibers . ''
	manualset3
89160	9	399721	5	NULL	NULL	0	NULL	Gasser	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1932 Sherrington and Adrian were awarded the Nobel Prize in Physiology or Medicine `` for their discoveries regarding the functions of neurons '' and in 1944 Erlanger and Gasser were awarded the same prize `` for their discoveries relating to the highly differentiated functions of single nerve fibers . ''
	manualset3
89161	10	399721	5	NULL	NULL	0	NULL	prize	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1932 Sherrington and Adrian were awarded the Nobel Prize in Physiology or Medicine `` for their discoveries regarding the functions of neurons '' and in 1944 Erlanger and Gasser were awarded the same prize `` for their discoveries relating to the highly differentiated functions of single nerve fibers . ''
	manualset3
89162	11	399721	5	NULL	NULL	0	NULL	highly differentiated functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1932 Sherrington and Adrian were awarded the Nobel Prize in Physiology or Medicine `` for their discoveries regarding the functions of neurons '' and in 1944 Erlanger and Gasser were awarded the same prize `` for their discoveries relating to the highly differentiated functions of single nerve fibers . ''
	manualset3
89163	12	399721	5	NULL	NULL	0	NULL	single nerve fibers	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1932 Sherrington and Adrian were awarded the Nobel Prize in Physiology or Medicine `` for their discoveries regarding the functions of neurons '' and in 1944 Erlanger and Gasser were awarded the same prize `` for their discoveries relating to the highly differentiated functions of single nerve fibers . ''
	manualset3
89164	1	399722	5	NULL	NULL	0	NULL	1986	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1986 the North Western Regional Health Authority ( RHA ) initiated the first large-scale attempt to use QALYs as a practical aid to planning in the National Health Service .
	manualset3
89165	2	399722	5	NULL	NULL	0	NULL	North Western Regional Health Authority ( RHA )	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1986 the North Western Regional Health Authority ( RHA ) initiated the first large-scale attempt to use QALYs as a practical aid to planning in the National Health Service .
	manualset3
89166	3	399722	5	NULL	NULL	0	NULL	first large-scale attempt	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1986 the North Western Regional Health Authority ( RHA ) initiated the first large-scale attempt to use QALYs as a practical aid to planning in the National Health Service .
	manualset3
89167	4	399722	5	NULL	NULL	0	NULL	QALYs	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1986 the North Western Regional Health Authority ( RHA ) initiated the first large-scale attempt to use QALYs as a practical aid to planning in the National Health Service .
	manualset3
89168	5	399722	5	NULL	NULL	0	NULL	practical aid	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1986 the North Western Regional Health Authority ( RHA ) initiated the first large-scale attempt to use QALYs as a practical aid to planning in the National Health Service .
	manualset3
89169	6	399722	5	NULL	NULL	0	NULL	National Health Service	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1986 the North Western Regional Health Authority ( RHA ) initiated the first large-scale attempt to use QALYs as a practical aid to planning in the National Health Service .
	manualset3
89170	1	399723	5	NULL	NULL	0	NULL	1993	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1993 each judicial district in Minnesota was told to create an organization to educate the community about child abuse and domestic violence .
	manualset3
89171	2	399723	5	NULL	NULL	0	NULL	judicial district in Minnesota	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1993 each judicial district in Minnesota was told to create an organization to educate the community about child abuse and domestic violence .
	manualset3
89172	3	399723	5	NULL	NULL	0	NULL	organization	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1993 each judicial district in Minnesota was told to create an organization to educate the community about child abuse and domestic violence .
	manualset3
89173	4	399723	5	NULL	NULL	0	NULL	community	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1993 each judicial district in Minnesota was told to create an organization to educate the community about child abuse and domestic violence .
	manualset3
89174	5	399723	5	NULL	NULL	NULL	NULL	child abuse	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In 1993 each judicial district in Minnesota was told to create an organization to educate the community about child abuse and domestic violence .
	manualset3
89175	6	399723	5	NULL	NULL	NULL	NULL	domestic violence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In 1993 each judicial district in Minnesota was told to create an organization to educate the community about child abuse and domestic violence .
	manualset3
89176	1	399724	5	NULL	NULL	0	NULL	20 eyes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In 20 eyes of 10 rabbits a siderosis was provoked by intravitreal injection of 0 , 1 ml of a 1 % watery solution of Mohr 's salt .
	manualset3
89177	2	399724	5	NULL	NULL	0	NULL	10 rabbits	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In 20 eyes of 10 rabbits a siderosis was provoked by intravitreal injection of 0 , 1 ml of a 1 % watery solution of Mohr 's salt .
	manualset3
89178	3	399724	5	NULL	NULL	0	NULL	siderosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 20 eyes of 10 rabbits a siderosis was provoked by intravitreal injection of 0 , 1 ml of a 1 % watery solution of Mohr 's salt .
	manualset3
89179	4	399724	5	NULL	NULL	0	NULL	 intravitreal injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 20 eyes of 10 rabbits a siderosis was provoked by intravitreal injection of 0 , 1 ml of a 1 % watery solution of Mohr 's salt .
	manualset3
89180	5	399724	5	NULL	NULL	0	NULL	0 , 1 ml of a 1 % watery solution of Mohr 's salt	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In 20 eyes of 10 rabbits a siderosis was provoked by intravitreal injection of 0 , 1 ml of a 1 % watery solution of Mohr 's salt .
	manualset3
89181	1	399725	5	NULL	NULL	0	NULL	20 h-old seedlings	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In 20 h-old seedlings , MTs in cortical cells destined to be a peg tissue had no preferential organization , whereas MTs in normal cortical cells were transversely oriented .
	manualset3
89182	2	399725	5	NULL	NULL	0	NULL	MTs	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In 20 h-old seedlings , MTs in cortical cells destined to be a peg tissue had no preferential organization , whereas MTs in normal cortical cells were transversely oriented .
	manualset3
89183	3	399725	5	NULL	NULL	0	NULL	cortical cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In 20 h-old seedlings , MTs in cortical cells destined to be a peg tissue had no preferential organization , whereas MTs in normal cortical cells were transversely oriented .
	manualset3
89184	4	399725	5	NULL	NULL	0	NULL	peg tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In 20 h-old seedlings , MTs in cortical cells destined to be a peg tissue had no preferential organization , whereas MTs in normal cortical cells were transversely oriented .
	manualset3
89185	5	399725	5	NULL	NULL	0	NULL	preferential organization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In 20 h-old seedlings , MTs in cortical cells destined to be a peg tissue had no preferential organization , whereas MTs in normal cortical cells were transversely oriented .
	manualset3
89186	6	399725	5	NULL	NULL	0	NULL	MTs	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In 20 h-old seedlings , MTs in cortical cells destined to be a peg tissue had no preferential organization , whereas MTs in normal cortical cells were transversely oriented .
	manualset3
89187	7	399725	5	NULL	NULL	0	NULL	normal cortical cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In 20 h-old seedlings , MTs in cortical cells destined to be a peg tissue had no preferential organization , whereas MTs in normal cortical cells were transversely oriented .
	manualset3
89188	1	399726	5	NULL	NULL	0	NULL	2000 to 2006	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In 2000 to 2006 , the female proportion increased in the structure of tuberculosis morbidity from 21.4 to 30.1 % and in that tuberculosis mortality from 13.1 to 21.4 % in the Sverdlovsk Region .
	manualset3
89189	2	399726	5	NULL	NULL	0	NULL	female proportion	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 2000 to 2006 , the female proportion increased in the structure of tuberculosis morbidity from 21.4 to 30.1 % and in that tuberculosis mortality from 13.1 to 21.4 % in the Sverdlovsk Region .
	manualset3
89190	3	399726	5	NULL	NULL	0	NULL	tuberculosis morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 2000 to 2006 , the female proportion increased in the structure of tuberculosis morbidity from 21.4 to 30.1 % and in that tuberculosis mortality from 13.1 to 21.4 % in the Sverdlovsk Region .
	manualset3
89191	4	399726	5	NULL	NULL	0	NULL	21.4 to 30.1 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In 2000 to 2006 , the female proportion increased in the structure of tuberculosis morbidity from 21.4 to 30.1 % and in that tuberculosis mortality from 13.1 to 21.4 % in the Sverdlovsk Region .
	manualset3
89192	5	399726	5	NULL	NULL	0	NULL	tuberculosis mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 2000 to 2006 , the female proportion increased in the structure of tuberculosis morbidity from 21.4 to 30.1 % and in that tuberculosis mortality from 13.1 to 21.4 % in the Sverdlovsk Region .
	manualset3
89193	6	399726	5	NULL	NULL	0	NULL	13.1 to 21.4 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In 2000 to 2006 , the female proportion increased in the structure of tuberculosis morbidity from 21.4 to 30.1 % and in that tuberculosis mortality from 13.1 to 21.4 % in the Sverdlovsk Region .
	manualset3
89194	7	399726	5	NULL	NULL	0	NULL	Sverdlovsk Region	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In 2000 to 2006 , the female proportion increased in the structure of tuberculosis morbidity from 21.4 to 30.1 % and in that tuberculosis mortality from 13.1 to 21.4 % in the Sverdlovsk Region .
	manualset3
89195	1	399727	5	NULL	NULL	0	NULL	2008	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	In 2008 19 subjects started treatment 3 weeks prior to the onset of birch pollen season in Ontario , Canada .
	manualset3
89196	2	399727	5	NULL	NULL	0	NULL	19 subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 2008 19 subjects started treatment 3 weeks prior to the onset of birch pollen season in Ontario , Canada .
	manualset3
89197	3	399727	5	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 2008 19 subjects started treatment 3 weeks prior to the onset of birch pollen season in Ontario , Canada .
	manualset3
89198	4	399727	5	NULL	NULL	0	NULL	3 weeks	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In 2008 19 subjects started treatment 3 weeks prior to the onset of birch pollen season in Ontario , Canada .
	manualset3
89199	5	399727	5	NULL	NULL	NULL	NULL	onset of birch pollen season	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In 2008 19 subjects started treatment 3 weeks prior to the onset of birch pollen season in Ontario , Canada .
	manualset3
89200	6	399727	5	NULL	NULL	0	NULL	Ontario , Canada	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In 2008 19 subjects started treatment 3 weeks prior to the onset of birch pollen season in Ontario , Canada .
	manualset3
89201	1	399728	5	NULL	NULL	0	NULL	21 episodes	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 21 episodes pathogens were isolated , 16 of them from the blood .
	manualset3
89202	2	399728	5	NULL	NULL	0	NULL	pathogens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In 21 episodes pathogens were isolated , 16 of them from the blood .
	manualset3
89203	3	399728	5	NULL	NULL	0	NULL	16	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In 21 episodes pathogens were isolated , 16 of them from the blood .
	manualset3
89204	4	399728	5	NULL	NULL	0	NULL	blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In 21 episodes pathogens were isolated , 16 of them from the blood .
	manualset3
89205	1	399729	5	NULL	NULL	0	NULL	24 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 24 patients undergoing elective coronary artery bypass grafting , plasma levels of interleukins IL-2 , IL-6 , IL-10 and IL-12 , soluble IL-2-receptor ( sIL-2R ) , and transforming growth factor-beta ( TGF-beta ) were measured at eight time points before , during and after CPB , using a standardized enzyme-linked immunosorbant assay technique .
	manualset3
89206	2	399729	5	NULL	NULL	0	NULL	elective coronary artery bypass grafting	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 24 patients undergoing elective coronary artery bypass grafting , plasma levels of interleukins IL-2 , IL-6 , IL-10 and IL-12 , soluble IL-2-receptor ( sIL-2R ) , and transforming growth factor-beta ( TGF-beta ) were measured at eight time points before , during and after CPB , using a standardized enzyme-linked immunosorbant assay technique .
	manualset3
89207	3	399729	5	NULL	NULL	0	NULL	plasma levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 24 patients undergoing elective coronary artery bypass grafting , plasma levels of interleukins IL-2 , IL-6 , IL-10 and IL-12 , soluble IL-2-receptor ( sIL-2R ) , and transforming growth factor-beta ( TGF-beta ) were measured at eight time points before , during and after CPB , using a standardized enzyme-linked immunosorbant assay technique .
	manualset3
89208	4	399729	5	NULL	NULL	0	NULL	interleukins IL-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In 24 patients undergoing elective coronary artery bypass grafting , plasma levels of interleukins IL-2 , IL-6 , IL-10 and IL-12 , soluble IL-2-receptor ( sIL-2R ) , and transforming growth factor-beta ( TGF-beta ) were measured at eight time points before , during and after CPB , using a standardized enzyme-linked immunosorbant assay technique .
	manualset3
89209	5	399729	5	NULL	NULL	0	NULL	IL-6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In 24 patients undergoing elective coronary artery bypass grafting , plasma levels of interleukins IL-2 , IL-6 , IL-10 and IL-12 , soluble IL-2-receptor ( sIL-2R ) , and transforming growth factor-beta ( TGF-beta ) were measured at eight time points before , during and after CPB , using a standardized enzyme-linked immunosorbant assay technique .
	manualset3
89210	6	399729	5	NULL	NULL	0	NULL	IL-10	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In 24 patients undergoing elective coronary artery bypass grafting , plasma levels of interleukins IL-2 , IL-6 , IL-10 and IL-12 , soluble IL-2-receptor ( sIL-2R ) , and transforming growth factor-beta ( TGF-beta ) were measured at eight time points before , during and after CPB , using a standardized enzyme-linked immunosorbant assay technique .
	manualset3
89211	7	399729	5	NULL	NULL	0	NULL	IL-12	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In 24 patients undergoing elective coronary artery bypass grafting , plasma levels of interleukins IL-2 , IL-6 , IL-10 and IL-12 , soluble IL-2-receptor ( sIL-2R ) , and transforming growth factor-beta ( TGF-beta ) were measured at eight time points before , during and after CPB , using a standardized enzyme-linked immunosorbant assay technique .
	manualset3
89212	8	399729	5	NULL	NULL	0	NULL	soluble IL-2-receptor ( sIL-2R )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In 24 patients undergoing elective coronary artery bypass grafting , plasma levels of interleukins IL-2 , IL-6 , IL-10 and IL-12 , soluble IL-2-receptor ( sIL-2R ) , and transforming growth factor-beta ( TGF-beta ) were measured at eight time points before , during and after CPB , using a standardized enzyme-linked immunosorbant assay technique .
	manualset3
89213	9	399729	5	NULL	NULL	0	NULL	transforming growth factor-beta ( TGF-beta )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In 24 patients undergoing elective coronary artery bypass grafting , plasma levels of interleukins IL-2 , IL-6 , IL-10 and IL-12 , soluble IL-2-receptor ( sIL-2R ) , and transforming growth factor-beta ( TGF-beta ) were measured at eight time points before , during and after CPB , using a standardized enzyme-linked immunosorbant assay technique .
	manualset3
89214	10	399729	5	NULL	NULL	0	NULL	eight time points	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 24 patients undergoing elective coronary artery bypass grafting , plasma levels of interleukins IL-2 , IL-6 , IL-10 and IL-12 , soluble IL-2-receptor ( sIL-2R ) , and transforming growth factor-beta ( TGF-beta ) were measured at eight time points before , during and after CPB , using a standardized enzyme-linked immunosorbant assay technique .
	manualset3
89215	11	399729	5	NULL	NULL	0	NULL	CPB	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 24 patients undergoing elective coronary artery bypass grafting , plasma levels of interleukins IL-2 , IL-6 , IL-10 and IL-12 , soluble IL-2-receptor ( sIL-2R ) , and transforming growth factor-beta ( TGF-beta ) were measured at eight time points before , during and after CPB , using a standardized enzyme-linked immunosorbant assay technique .
	manualset3
89216	12	399729	5	NULL	NULL	0	NULL	standardized enzyme-linked immunosorbant assay technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 24 patients undergoing elective coronary artery bypass grafting , plasma levels of interleukins IL-2 , IL-6 , IL-10 and IL-12 , soluble IL-2-receptor ( sIL-2R ) , and transforming growth factor-beta ( TGF-beta ) were measured at eight time points before , during and after CPB , using a standardized enzyme-linked immunosorbant assay technique .
	manualset3
89217	1	399730	5	NULL	NULL	0	NULL	259 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 259 patients with conduction disturbances , 76 ( 2.3 % ) had indeterminate ventricular conduction disturbances , 126 ( 3.8 % ) had right bundle branch block , and 47 ( 1.4 % ) had left bundle branch block .
	manualset3
89218	2	399730	5	NULL	NULL	0	NULL	conduction disturbances	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 259 patients with conduction disturbances , 76 ( 2.3 % ) had indeterminate ventricular conduction disturbances , 126 ( 3.8 % ) had right bundle branch block , and 47 ( 1.4 % ) had left bundle branch block .
	manualset3
89219	3	399730	5	NULL	NULL	0	NULL	76 ( 2.3 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In 259 patients with conduction disturbances , 76 ( 2.3 % ) had indeterminate ventricular conduction disturbances , 126 ( 3.8 % ) had right bundle branch block , and 47 ( 1.4 % ) had left bundle branch block .
	manualset3
89220	4	399730	5	NULL	NULL	0	NULL	indeterminate ventricular conduction disturbances	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 259 patients with conduction disturbances , 76 ( 2.3 % ) had indeterminate ventricular conduction disturbances , 126 ( 3.8 % ) had right bundle branch block , and 47 ( 1.4 % ) had left bundle branch block .
	manualset3
89221	5	399730	5	NULL	NULL	0	NULL	126 ( 3.8 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In 259 patients with conduction disturbances , 76 ( 2.3 % ) had indeterminate ventricular conduction disturbances , 126 ( 3.8 % ) had right bundle branch block , and 47 ( 1.4 % ) had left bundle branch block .
	manualset3
89222	6	399730	5	NULL	NULL	0	NULL	right bundle branch block	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 259 patients with conduction disturbances , 76 ( 2.3 % ) had indeterminate ventricular conduction disturbances , 126 ( 3.8 % ) had right bundle branch block , and 47 ( 1.4 % ) had left bundle branch block .
	manualset3
89223	7	399730	5	NULL	NULL	0	NULL	47 ( 1.4 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In 259 patients with conduction disturbances , 76 ( 2.3 % ) had indeterminate ventricular conduction disturbances , 126 ( 3.8 % ) had right bundle branch block , and 47 ( 1.4 % ) had left bundle branch block .
	manualset3
89224	8	399730	5	NULL	NULL	0	NULL	left bundle branch block 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 259 patients with conduction disturbances , 76 ( 2.3 % ) had indeterminate ventricular conduction disturbances , 126 ( 3.8 % ) had right bundle branch block , and 47 ( 1.4 % ) had left bundle branch block .
	manualset3
89311	1	399731	5	NULL	NULL	0	NULL	271 Enterobacter blood culture isolates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In 271 Enterobacter blood culture isolates from 12 hospitals , extended-spectrum beta-lactamase ( ESBL ) prevalence varied between 0 % and 30 % per hospital .
	manualset3
89312	2	399731	5	NULL	NULL	0	NULL	12 hospitals	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In 271 Enterobacter blood culture isolates from 12 hospitals , extended-spectrum beta-lactamase ( ESBL ) prevalence varied between 0 % and 30 % per hospital .
	manualset3
89313	3	399731	5	NULL	NULL	0	NULL	extended-spectrum beta-lactamase ( ESBL ) prevalence	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In 271 Enterobacter blood culture isolates from 12 hospitals , extended-spectrum beta-lactamase ( ESBL ) prevalence varied between 0 % and 30 % per hospital .
	manualset3
89314	4	399731	5	NULL	NULL	0	NULL	 0 % and 30 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In 271 Enterobacter blood culture isolates from 12 hospitals , extended-spectrum beta-lactamase ( ESBL ) prevalence varied between 0 % and 30 % per hospital .
	manualset3
89315	5	399731	5	NULL	NULL	0	NULL	hospital	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In 271 Enterobacter blood culture isolates from 12 hospitals , extended-spectrum beta-lactamase ( ESBL ) prevalence varied between 0 % and 30 % per hospital .
	manualset3
89316	1	399732	5	NULL	NULL	0	NULL	29 of 36 children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 29 of 36 children with fetal alcohol syndrome brainstem auditory-evoked potentials were performed and the auditory threshold was determined .
	manualset3
89317	2	399732	5	NULL	NULL	0	NULL	fetal alcohol syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In 29 of 36 children with fetal alcohol syndrome brainstem auditory-evoked potentials were performed and the auditory threshold was determined .
	manualset3
89318	3	399732	5	NULL	NULL	0	NULL	brainstem auditory-evoked potentials	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 29 of 36 children with fetal alcohol syndrome brainstem auditory-evoked potentials were performed and the auditory threshold was determined .
	manualset3
89319	4	399732	5	NULL	NULL	0	NULL	auditory threshold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 29 of 36 children with fetal alcohol syndrome brainstem auditory-evoked potentials were performed and the auditory threshold was determined .
	manualset3
89320	1	399733	5	NULL	NULL	0	NULL	49 consecutive patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 49 consecutive patients ( 27 men and 22 women , age range 44 to 86 years ) presenting with acute symptoms and with subsequently proven pulmonary embolism , and without previous lung disease , the 12-lead electrocardiograms obtained at hospital admission were reviewed in a blinded fashion to identify electrocardiographic features suggestive of right ventricular overload .
	manualset3
89321	2	399733	5	NULL	NULL	0	NULL	27 men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 49 consecutive patients ( 27 men and 22 women , age range 44 to 86 years ) presenting with acute symptoms and with subsequently proven pulmonary embolism , and without previous lung disease , the 12-lead electrocardiograms obtained at hospital admission were reviewed in a blinded fashion to identify electrocardiographic features suggestive of right ventricular overload .
	manualset3
89322	3	399733	5	NULL	NULL	0	NULL	22 women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 49 consecutive patients ( 27 men and 22 women , age range 44 to 86 years ) presenting with acute symptoms and with subsequently proven pulmonary embolism , and without previous lung disease , the 12-lead electrocardiograms obtained at hospital admission were reviewed in a blinded fashion to identify electrocardiographic features suggestive of right ventricular overload .
	manualset3
89324	4	399733	5	NULL	NULL	0	NULL	age range 44 to 86 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In 49 consecutive patients ( 27 men and 22 women , age range 44 to 86 years ) presenting with acute symptoms and with subsequently proven pulmonary embolism , and without previous lung disease , the 12-lead electrocardiograms obtained at hospital admission were reviewed in a blinded fashion to identify electrocardiographic features suggestive of right ventricular overload .
	manualset3
89326	5	399733	5	NULL	NULL	0	NULL	acute symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 49 consecutive patients ( 27 men and 22 women , age range 44 to 86 years ) presenting with acute symptoms and with subsequently proven pulmonary embolism , and without previous lung disease , the 12-lead electrocardiograms obtained at hospital admission were reviewed in a blinded fashion to identify electrocardiographic features suggestive of right ventricular overload .
	manualset3
89329	6	399733	5	NULL	NULL	0	NULL	subsequently proven pulmonary embolism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 49 consecutive patients ( 27 men and 22 women , age range 44 to 86 years ) presenting with acute symptoms and with subsequently proven pulmonary embolism , and without previous lung disease , the 12-lead electrocardiograms obtained at hospital admission were reviewed in a blinded fashion to identify electrocardiographic features suggestive of right ventricular overload .
	manualset3
89330	7	399733	5	NULL	NULL	0	NULL	lung disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In 49 consecutive patients ( 27 men and 22 women , age range 44 to 86 years ) presenting with acute symptoms and with subsequently proven pulmonary embolism , and without previous lung disease , the 12-lead electrocardiograms obtained at hospital admission were reviewed in a blinded fashion to identify electrocardiographic features suggestive of right ventricular overload .
	manualset3
89331	8	399733	5	NULL	NULL	0	NULL	12-lead electrocardiograms	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 49 consecutive patients ( 27 men and 22 women , age range 44 to 86 years ) presenting with acute symptoms and with subsequently proven pulmonary embolism , and without previous lung disease , the 12-lead electrocardiograms obtained at hospital admission were reviewed in a blinded fashion to identify electrocardiographic features suggestive of right ventricular overload .
	manualset3
89332	9	399733	5	NULL	NULL	0	NULL	hospital admission	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 49 consecutive patients ( 27 men and 22 women , age range 44 to 86 years ) presenting with acute symptoms and with subsequently proven pulmonary embolism , and without previous lung disease , the 12-lead electrocardiograms obtained at hospital admission were reviewed in a blinded fashion to identify electrocardiographic features suggestive of right ventricular overload .
	manualset3
89333	10	399733	5	NULL	NULL	0	NULL	electrocardiographic features	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 49 consecutive patients ( 27 men and 22 women , age range 44 to 86 years ) presenting with acute symptoms and with subsequently proven pulmonary embolism , and without previous lung disease , the 12-lead electrocardiograms obtained at hospital admission were reviewed in a blinded fashion to identify electrocardiographic features suggestive of right ventricular overload .
	manualset3
89334	11	399733	5	NULL	NULL	0	NULL	right ventricular overload	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 49 consecutive patients ( 27 men and 22 women , age range 44 to 86 years ) presenting with acute symptoms and with subsequently proven pulmonary embolism , and without previous lung disease , the 12-lead electrocardiograms obtained at hospital admission were reviewed in a blinded fashion to identify electrocardiographic features suggestive of right ventricular overload .
	manualset3
89335	1	399734	5	NULL	NULL	0	NULL	496 subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 496 subjects , the NADPH oxidase-dependent superoxide production in peripheral blood mononuclear cells was assessed by chemiluminescence .
	manualset3
89336	2	399734	5	NULL	NULL	0	NULL	NADPH oxidase-dependent superoxide production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In 496 subjects , the NADPH oxidase-dependent superoxide production in peripheral blood mononuclear cells was assessed by chemiluminescence .
	manualset3
89338	3	399734	5	NULL	NULL	0	NULL	peripheral blood mononuclear cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In 496 subjects , the NADPH oxidase-dependent superoxide production in peripheral blood mononuclear cells was assessed by chemiluminescence .
	manualset3
89339	4	399734	5	NULL	NULL	0	NULL	chemiluminescence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 496 subjects , the NADPH oxidase-dependent superoxide production in peripheral blood mononuclear cells was assessed by chemiluminescence .
	manualset3
89340	1	399735	5	NULL	NULL	0	NULL	15 cases ( 33 % ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In 5 of the 15 cases ( 33 % ) , p53 gene mutation was identified and these tumors were subsequently histologically diagnosed as malignant .
	manualset3
89342	2	399735	5	NULL	NULL	0	NULL	p53 gene mutation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In 5 of the 15 cases ( 33 % ) , p53 gene mutation was identified and these tumors were subsequently histologically diagnosed as malignant .
	manualset3
89346	3	399735	5	NULL	NULL	0	NULL	tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 5 of the 15 cases ( 33 % ) , p53 gene mutation was identified and these tumors were subsequently histologically diagnosed as malignant .
	manualset3
89355	1	399736	5	NULL	NULL	0	NULL	lymphocytes-macrophage interaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In 5 of them a lymphocytes-macrophage interaction ( `` immunological island '' ) was found : these 5 patients responded well to chemotherapy and their clinical course was satisfactory .
	manualset3
89363	2	399736	5	NULL	NULL	0	NULL	immunological island	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 5 of them a lymphocytes-macrophage interaction ( `` immunological island '' ) was found : these 5 patients responded well to chemotherapy and their clinical course was satisfactory .
	manualset3
89366	3	399736	5	NULL	NULL	0	NULL	5 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 5 of them a lymphocytes-macrophage interaction ( `` immunological island '' ) was found : these 5 patients responded well to chemotherapy and their clinical course was satisfactory .
	manualset3
89367	4	399736	5	NULL	NULL	0	NULL	chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 5 of them a lymphocytes-macrophage interaction ( `` immunological island '' ) was found : these 5 patients responded well to chemotherapy and their clinical course was satisfactory .
	manualset3
89368	5	399736	5	NULL	NULL	0	NULL	clinical course	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 5 of them a lymphocytes-macrophage interaction ( `` immunological island '' ) was found : these 5 patients responded well to chemotherapy and their clinical course was satisfactory .
	manualset3
89369	1	399737	5	NULL	NULL	0	NULL	7 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 7 patients , mean daily serum GH decreased but not to normal ; 3 of these patients had hyperprolactinemia which was not influenced by octreotide .
	manualset3
89370	2	399737	5	NULL	NULL	0	NULL	mean daily serum GH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In 7 patients , mean daily serum GH decreased but not to normal ; 3 of these patients had hyperprolactinemia which was not influenced by octreotide .
	manualset3
89372	3	399737	5	NULL	NULL	NULL	NULL	3 of these patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In 7 patients , mean daily serum GH decreased but not to normal ; 3 of these patients had hyperprolactinemia which was not influenced by octreotide .
	manualset3
89373	4	399737	5	NULL	NULL	NULL	NULL	hyperprolactinemia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In 7 patients , mean daily serum GH decreased but not to normal ; 3 of these patients had hyperprolactinemia which was not influenced by octreotide .
	manualset3
89374	5	399737	5	NULL	NULL	NULL	NULL	octreotide	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In 7 patients , mean daily serum GH decreased but not to normal ; 3 of these patients had hyperprolactinemia which was not influenced by octreotide .
	manualset3
89375	1	399738	5	NULL	NULL	0	NULL	70 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 70 patients , a cytopathologic diagnosis of atypical metaplasia was made .
	manualset3
89376	2	399738	5	NULL	NULL	0	NULL	cytopathologic diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 70 patients , a cytopathologic diagnosis of atypical metaplasia was made .
	manualset3
89377	3	399738	5	NULL	NULL	0	NULL	atypical metaplasia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In 70 patients , a cytopathologic diagnosis of atypical metaplasia was made .
	manualset3
89378	1	399739	5	NULL	NULL	0	NULL	74 cases ( 69.8 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In 74 cases ( 69.8 % ) the corneal scar was either transparent or discrete , whilst in 32 cases ( 30.2 % ) a mild or marked scar was observed .
	manualset3
89379	2	399739	5	NULL	NULL	0	NULL	corneal scar	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 74 cases ( 69.8 % ) the corneal scar was either transparent or discrete , whilst in 32 cases ( 30.2 % ) a mild or marked scar was observed .
	manualset3
89381	3	399739	5	NULL	NULL	NULL	NULL	32 cases ( 30.2 % )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In 74 cases ( 69.8 % ) the corneal scar was either transparent or discrete , whilst in 32 cases ( 30.2 % ) a mild or marked scar was observed .
	manualset3
89382	4	399739	5	NULL	NULL	NULL	NULL	mild or marked scar	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In 74 cases ( 69.8 % ) the corneal scar was either transparent or discrete , whilst in 32 cases ( 30.2 % ) a mild or marked scar was observed .
	manualset3
89384	1	399740	5	NULL	NULL	0	NULL	bilharziasis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In 8 of these , bilharziasis of the rectum and colon was found to be the cause of the prolapse .
	manualset3
89385	2	399740	5	NULL	NULL	0	NULL	rectum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In 8 of these , bilharziasis of the rectum and colon was found to be the cause of the prolapse .
	manualset3
89386	3	399740	5	NULL	NULL	0	NULL	colon	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In 8 of these , bilharziasis of the rectum and colon was found to be the cause of the prolapse .
	manualset3
89389	4	399740	5	NULL	NULL	0	NULL	prolapse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 8 of these , bilharziasis of the rectum and colon was found to be the cause of the prolapse .
	manualset3
89394	1	399741	5	NULL	NULL	NULL	NULL	8 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In 8 patients ( 6.0 % ) , no antileukemic therapy at all was given ( either they died shortly after admission to the ward or therapy was not feasible due to their clinical status ) .
	manualset3
89396	2	399741	5	NULL	NULL	0	NULL	antileukemic therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 8 patients ( 6.0 % ) , no antileukemic therapy at all was given ( either they died shortly after admission to the ward or therapy was not feasible due to their clinical status ) .
	manualset3
89397	3	399741	5	NULL	NULL	0	NULL	admission	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 8 patients ( 6.0 % ) , no antileukemic therapy at all was given ( either they died shortly after admission to the ward or therapy was not feasible due to their clinical status ) .
	manualset3
89399	4	399741	5	NULL	NULL	0	NULL	ward	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In 8 patients ( 6.0 % ) , no antileukemic therapy at all was given ( either they died shortly after admission to the ward or therapy was not feasible due to their clinical status ) .
	manualset3
89400	5	399741	5	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 8 patients ( 6.0 % ) , no antileukemic therapy at all was given ( either they died shortly after admission to the ward or therapy was not feasible due to their clinical status ) .
	manualset3
89403	6	399741	5	NULL	NULL	0	NULL	clinical status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 8 patients ( 6.0 % ) , no antileukemic therapy at all was given ( either they died shortly after admission to the ward or therapy was not feasible due to their clinical status ) .
	manualset3
92571	7	399741	5	NULL	NULL	0	NULL	 ( 6.0 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In 8 patients ( 6.0 % ) , no antileukemic therapy at all was given ( either they died shortly after admission to the ward or therapy was not feasible due to their clinical status ) .
	manualset3
89405	1	399742	5	NULL	NULL	0	NULL	80 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In 80 % one relative was affected , in most cases a first-degree relative with UC .
	manualset3
89406	2	399742	5	NULL	NULL	0	NULL	relative	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In 80 % one relative was affected , in most cases a first-degree relative with UC .
	manualset3
89414	3	399742	5	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 80 % one relative was affected , in most cases a first-degree relative with UC .
	manualset3
89416	4	399742	5	NULL	NULL	0	NULL	first-degree relative	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In 80 % one relative was affected , in most cases a first-degree relative with UC .
	manualset3
89419	5	399742	5	NULL	NULL	0	NULL	UC	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 80 % one relative was affected , in most cases a first-degree relative with UC .
	manualset3
89421	1	399743	5	NULL	NULL	0	NULL	84 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In 84 % of all patients , movement of the SIJ was restricted .
	manualset3
89422	2	399743	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 84 % of all patients , movement of the SIJ was restricted .
	manualset3
89423	3	399743	5	NULL	NULL	0	NULL	movement of the SIJ	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In 84 % of all patients , movement of the SIJ was restricted .
	manualset3
89430	1	399744	5	NULL	NULL	0	NULL	APEC O78 strain chi7122	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In APEC O78 strain chi7122 , a functional Pst system is required for full virulence and resistance to acid shock and polymyxin .
	manualset3
89432	2	399744	5	NULL	NULL	NULL	NULL	functional Pst system	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In APEC O78 strain chi7122 , a functional Pst system is required for full virulence and resistance to acid shock and polymyxin .
	manualset3
89435	3	399744	5	NULL	NULL	0	NULL	full virulence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In APEC O78 strain chi7122 , a functional Pst system is required for full virulence and resistance to acid shock and polymyxin .
	manualset3
89436	4	399744	5	NULL	NULL	0	NULL	resistance to acid shock	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In APEC O78 strain chi7122 , a functional Pst system is required for full virulence and resistance to acid shock and polymyxin .
	manualset3
89439	5	399744	5	NULL	NULL	NULL	NULL	polymyxin 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In APEC O78 strain chi7122 , a functional Pst system is required for full virulence and resistance to acid shock and polymyxin .
	manualset3
89442	1	399745	5	NULL	NULL	0	NULL	AdCMVeNOS basilar arteries with endothelium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In AdCMVeNOS basilar arteries with endothelium , relaxations to low concentrations of bradykinin ( 3 x 10 ( -11 ) to 10 ( -9 ) mol/L ) were significantly augmented .
	manualset3
89445	2	399745	5	NULL	NULL	0	NULL	relaxations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In AdCMVeNOS basilar arteries with endothelium , relaxations to low concentrations of bradykinin ( 3 x 10 ( -11 ) to 10 ( -9 ) mol/L ) were significantly augmented .
	manualset3
89446	3	399745	5	NULL	NULL	0	NULL	low concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In AdCMVeNOS basilar arteries with endothelium , relaxations to low concentrations of bradykinin ( 3 x 10 ( -11 ) to 10 ( -9 ) mol/L ) were significantly augmented .
	manualset3
89452	4	399745	5	NULL	NULL	0	NULL	bradykinin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In AdCMVeNOS basilar arteries with endothelium , relaxations to low concentrations of bradykinin ( 3 x 10 ( -11 ) to 10 ( -9 ) mol/L ) were significantly augmented .
	manualset3
89453	5	399745	5	NULL	NULL	0	NULL	( 3 x 10 ( -11 ) to 10 ( -9 ) mol/L )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In AdCMVeNOS basilar arteries with endothelium , relaxations to low concentrations of bradykinin ( 3 x 10 ( -11 ) to 10 ( -9 ) mol/L ) were significantly augmented .
	manualset3
89454	1	399746	5	NULL	NULL	0	NULL	Arabidopsis thaliana	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In Arabidopsis thaliana , two AUXIN RESPONSE FACTORs ( ARFs ) , ARF7 and ARF19 , positively regulate LR formation through activation of the plant-specific transcriptional regulators LATERAL ORGAN BOUNDARIES-DOMAIN 16/ASYMMETRIC LEAVES2-LIKE 18 ( LBD16/ASL18 ) and the other related LBD/ASL genes .
	manualset3
89456	2	399746	5	NULL	NULL	0	NULL	AUXIN RESPONSE FACTORs ( ARFs )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In Arabidopsis thaliana , two AUXIN RESPONSE FACTORs ( ARFs ) , ARF7 and ARF19 , positively regulate LR formation through activation of the plant-specific transcriptional regulators LATERAL ORGAN BOUNDARIES-DOMAIN 16/ASYMMETRIC LEAVES2-LIKE 18 ( LBD16/ASL18 ) and the other related LBD/ASL genes .
	manualset3
89458	3	399746	5	NULL	NULL	0	NULL	ARF7	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In Arabidopsis thaliana , two AUXIN RESPONSE FACTORs ( ARFs ) , ARF7 and ARF19 , positively regulate LR formation through activation of the plant-specific transcriptional regulators LATERAL ORGAN BOUNDARIES-DOMAIN 16/ASYMMETRIC LEAVES2-LIKE 18 ( LBD16/ASL18 ) and the other related LBD/ASL genes .
	manualset3
89459	4	399746	5	NULL	NULL	0	NULL	ARF19	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In Arabidopsis thaliana , two AUXIN RESPONSE FACTORs ( ARFs ) , ARF7 and ARF19 , positively regulate LR formation through activation of the plant-specific transcriptional regulators LATERAL ORGAN BOUNDARIES-DOMAIN 16/ASYMMETRIC LEAVES2-LIKE 18 ( LBD16/ASL18 ) and the other related LBD/ASL genes .
	manualset3
89462	5	399746	5	NULL	NULL	0	NULL	LR formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In Arabidopsis thaliana , two AUXIN RESPONSE FACTORs ( ARFs ) , ARF7 and ARF19 , positively regulate LR formation through activation of the plant-specific transcriptional regulators LATERAL ORGAN BOUNDARIES-DOMAIN 16/ASYMMETRIC LEAVES2-LIKE 18 ( LBD16/ASL18 ) and the other related LBD/ASL genes .
	manualset3
89465	6	399746	5	NULL	NULL	0	NULL	activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In Arabidopsis thaliana , two AUXIN RESPONSE FACTORs ( ARFs ) , ARF7 and ARF19 , positively regulate LR formation through activation of the plant-specific transcriptional regulators LATERAL ORGAN BOUNDARIES-DOMAIN 16/ASYMMETRIC LEAVES2-LIKE 18 ( LBD16/ASL18 ) and the other related LBD/ASL genes .
	manualset3
89467	7	399746	5	NULL	NULL	0	NULL	plant-specific transcriptional regulators	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In Arabidopsis thaliana , two AUXIN RESPONSE FACTORs ( ARFs ) , ARF7 and ARF19 , positively regulate LR formation through activation of the plant-specific transcriptional regulators LATERAL ORGAN BOUNDARIES-DOMAIN 16/ASYMMETRIC LEAVES2-LIKE 18 ( LBD16/ASL18 ) and the other related LBD/ASL genes .
	manualset3
89468	8	399746	5	NULL	NULL	0	NULL	LATERAL ORGAN BOUNDARIES-DOMAIN 16/ASYMMETRIC LEAVES2-LIKE 18 ( LBD16/ASL18 )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In Arabidopsis thaliana , two AUXIN RESPONSE FACTORs ( ARFs ) , ARF7 and ARF19 , positively regulate LR formation through activation of the plant-specific transcriptional regulators LATERAL ORGAN BOUNDARIES-DOMAIN 16/ASYMMETRIC LEAVES2-LIKE 18 ( LBD16/ASL18 ) and the other related LBD/ASL genes .
	manualset3
89469	9	399746	5	NULL	NULL	NULL	NULL	other related LBD/ASL genes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In Arabidopsis thaliana , two AUXIN RESPONSE FACTORs ( ARFs ) , ARF7 and ARF19 , positively regulate LR formation through activation of the plant-specific transcriptional regulators LATERAL ORGAN BOUNDARIES-DOMAIN 16/ASYMMETRIC LEAVES2-LIKE 18 ( LBD16/ASL18 ) and the other related LBD/ASL genes .
	manualset3
89470	1	399747	5	NULL	NULL	0	NULL	Arabidopsis plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In Arabidopsis plants defective in the - subunit of the AP-3 adaptor complex , INT1 is correctly localized to the tonoplast , while sorting of the vacuolar sucrose transporter SUC4 is blocked in cis-Golgi stacks .
	manualset3
89471	2	399747	5	NULL	NULL	0	NULL	subunit of the AP-3 adaptor complex , INT1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In Arabidopsis plants defective in the - subunit of the AP-3 adaptor complex , INT1 is correctly localized to the tonoplast , while sorting of the vacuolar sucrose transporter SUC4 is blocked in cis-Golgi stacks .
	manualset3
89472	3	399747	5	NULL	NULL	0	NULL	tonoplast	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In Arabidopsis plants defective in the - subunit of the AP-3 adaptor complex , INT1 is correctly localized to the tonoplast , while sorting of the vacuolar sucrose transporter SUC4 is blocked in cis-Golgi stacks .
	manualset3
89473	4	399747	5	NULL	NULL	0	NULL	vacuolar sucrose transporter SUC4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In Arabidopsis plants defective in the - subunit of the AP-3 adaptor complex , INT1 is correctly localized to the tonoplast , while sorting of the vacuolar sucrose transporter SUC4 is blocked in cis-Golgi stacks .
	manualset3
89475	5	399747	5	NULL	NULL	0	NULL	cis-Golgi stacks	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In Arabidopsis plants defective in the - subunit of the AP-3 adaptor complex , INT1 is correctly localized to the tonoplast , while sorting of the vacuolar sucrose transporter SUC4 is blocked in cis-Golgi stacks .
	manualset3
89477	1	399748	5	NULL	NULL	0	NULL	August 2011	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	In August 2011 , scientists and policy-makers held a conference entitled `` Using IT to Improve Community Health : How Health Care Reform Supports Innovation . ''
	manualset3
89478	2	399748	5	NULL	NULL	0	NULL	scientists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In August 2011 , scientists and policy-makers held a conference entitled `` Using IT to Improve Community Health : How Health Care Reform Supports Innovation . ''
	manualset3
89479	3	399748	5	NULL	NULL	0	NULL	policy-makers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In August 2011 , scientists and policy-makers held a conference entitled `` Using IT to Improve Community Health : How Health Care Reform Supports Innovation . ''
	manualset3
89480	4	399748	5	NULL	NULL	0	NULL	conference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In August 2011 , scientists and policy-makers held a conference entitled `` Using IT to Improve Community Health : How Health Care Reform Supports Innovation . ''
	manualset3
89483	5	399748	5	NULL	NULL	0	NULL	IT	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In August 2011 , scientists and policy-makers held a conference entitled `` Using IT to Improve Community Health : How Health Care Reform Supports Innovation . ''
	manualset3
89484	6	399748	5	NULL	NULL	0	NULL	Community Health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In August 2011 , scientists and policy-makers held a conference entitled `` Using IT to Improve Community Health : How Health Care Reform Supports Innovation . ''
	manualset3
89485	7	399748	5	NULL	NULL	0	NULL	Health Care Reform	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In August 2011 , scientists and policy-makers held a conference entitled `` Using IT to Improve Community Health : How Health Care Reform Supports Innovation . ''
	manualset3
89486	8	399748	5	NULL	NULL	0	NULL	Innovation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In August 2011 , scientists and policy-makers held a conference entitled `` Using IT to Improve Community Health : How Health Care Reform Supports Innovation . ''
	manualset3
89489	1	399749	5	NULL	NULL	0	NULL	B. abortus-immunized birds	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In B. abortus-immunized birds , sex x line interactions indicated that males of the HL and CL had lower responses than females but LL males were not different than females .
	manualset3
89490	2	399749	5	NULL	NULL	0	NULL	sex x line interactions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In B. abortus-immunized birds , sex x line interactions indicated that males of the HL and CL had lower responses than females but LL males were not different than females .
	manualset3
89492	3	399749	5	NULL	NULL	0	NULL	males	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In B. abortus-immunized birds , sex x line interactions indicated that males of the HL and CL had lower responses than females but LL males were not different than females .
	manualset3
89631	4	399749	5	NULL	NULL	0	NULL	HL	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In B. abortus-immunized birds , sex x line interactions indicated that males of the HL and CL had lower responses than females but LL males were not different than females .
	manualset3
89632	5	399749	5	NULL	NULL	0	NULL	CL	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In B. abortus-immunized birds , sex x line interactions indicated that males of the HL and CL had lower responses than females but LL males were not different than females .
	manualset3
89633	6	399749	5	NULL	NULL	0	NULL	lower responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In B. abortus-immunized birds , sex x line interactions indicated that males of the HL and CL had lower responses than females but LL males were not different than females .
	manualset3
89634	7	399749	5	NULL	NULL	0	NULL	females	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In B. abortus-immunized birds , sex x line interactions indicated that males of the HL and CL had lower responses than females but LL males were not different than females .
	manualset3
89635	8	399749	5	NULL	NULL	0	NULL	LL males	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In B. abortus-immunized birds , sex x line interactions indicated that males of the HL and CL had lower responses than females but LL males were not different than females .
	manualset3
89636	9	399749	5	NULL	NULL	0	NULL	females	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In B. abortus-immunized birds , sex x line interactions indicated that males of the HL and CL had lower responses than females but LL males were not different than females .
	manualset3
89637	1	399750	5	NULL	NULL	0	NULL	CAPD	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In CAPD decreased blood concentrations of some water soluble vitamins are found due to insufficient dietary intake and loss into dialyzate .
	manualset3
89638	2	399750	5	NULL	NULL	0	NULL	decreased blood concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In CAPD decreased blood concentrations of some water soluble vitamins are found due to insufficient dietary intake and loss into dialyzate .
	manualset3
89639	3	399750	5	NULL	NULL	0	NULL	water soluble vitamins	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In CAPD decreased blood concentrations of some water soluble vitamins are found due to insufficient dietary intake and loss into dialyzate .
	manualset3
89640	4	399750	5	NULL	NULL	0	NULL	insufficient dietary intake	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In CAPD decreased blood concentrations of some water soluble vitamins are found due to insufficient dietary intake and loss into dialyzate .
	manualset3
89641	5	399750	5	NULL	NULL	0	NULL	loss into dialyzate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In CAPD decreased blood concentrations of some water soluble vitamins are found due to insufficient dietary intake and loss into dialyzate .
	manualset3
89642	1	399751	5	NULL	NULL	0	NULL	COS-1 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In COS-1 cells , US28 was expressed on the cell surface and could mediate cell-cell fusion with HIV-1 Env-expressing cells , suggesting that the block to infection may result from a defect in virus internalization or postentry steps .
	manualset3
89643	2	399751	5	NULL	NULL	0	NULL	US28	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In COS-1 cells , US28 was expressed on the cell surface and could mediate cell-cell fusion with HIV-1 Env-expressing cells , suggesting that the block to infection may result from a defect in virus internalization or postentry steps .
	manualset3
89645	3	399751	5	NULL	NULL	0	NULL	cell surface	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In COS-1 cells , US28 was expressed on the cell surface and could mediate cell-cell fusion with HIV-1 Env-expressing cells , suggesting that the block to infection may result from a defect in virus internalization or postentry steps .
	manualset3
89646	4	399751	5	NULL	NULL	0	NULL	cell-cell fusion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In COS-1 cells , US28 was expressed on the cell surface and could mediate cell-cell fusion with HIV-1 Env-expressing cells , suggesting that the block to infection may result from a defect in virus internalization or postentry steps .
	manualset3
89647	5	399751	5	NULL	NULL	0	NULL	HIV-1 Env-expressing cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In COS-1 cells , US28 was expressed on the cell surface and could mediate cell-cell fusion with HIV-1 Env-expressing cells , suggesting that the block to infection may result from a defect in virus internalization or postentry steps .
	manualset3
89656	6	399751	5	NULL	NULL	0	NULL	block to infection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In COS-1 cells , US28 was expressed on the cell surface and could mediate cell-cell fusion with HIV-1 Env-expressing cells , suggesting that the block to infection may result from a defect in virus internalization or postentry steps .
	manualset3
89657	7	399751	5	NULL	NULL	0	NULL	defect in virus internalization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In COS-1 cells , US28 was expressed on the cell surface and could mediate cell-cell fusion with HIV-1 Env-expressing cells , suggesting that the block to infection may result from a defect in virus internalization or postentry steps .
	manualset3
89658	8	399751	5	NULL	NULL	0	NULL	postentry steps	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In COS-1 cells , US28 was expressed on the cell surface and could mediate cell-cell fusion with HIV-1 Env-expressing cells , suggesting that the block to infection may result from a defect in virus internalization or postentry steps .
	manualset3
89660	1	399752	5	NULL	NULL	0	NULL	Caenorhabditis elegans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In Caenorhabditis elegans the polyamine synthetic pathway consists of three enzymes , ornithine decarboxylase ( ODC ) , S-adenosylmethionine decarboxylase ( AdoMetDC ) and spermidine synthase .
	manualset3
89661	2	399752	5	NULL	NULL	0	NULL	polyamine synthetic pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In Caenorhabditis elegans the polyamine synthetic pathway consists of three enzymes , ornithine decarboxylase ( ODC ) , S-adenosylmethionine decarboxylase ( AdoMetDC ) and spermidine synthase .
	manualset3
89662	3	399752	5	NULL	NULL	NULL	NULL	three enzymes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In Caenorhabditis elegans the polyamine synthetic pathway consists of three enzymes , ornithine decarboxylase ( ODC ) , S-adenosylmethionine decarboxylase ( AdoMetDC ) and spermidine synthase .
	manualset3
89663	4	399752	5	NULL	NULL	0	NULL	ornithine decarboxylase ( ODC )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In Caenorhabditis elegans the polyamine synthetic pathway consists of three enzymes , ornithine decarboxylase ( ODC ) , S-adenosylmethionine decarboxylase ( AdoMetDC ) and spermidine synthase .
	manualset3
89664	5	399752	5	NULL	NULL	0	NULL	S-adenosylmethionine decarboxylase ( AdoMetDC )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In Caenorhabditis elegans the polyamine synthetic pathway consists of three enzymes , ornithine decarboxylase ( ODC ) , S-adenosylmethionine decarboxylase ( AdoMetDC ) and spermidine synthase .
	manualset3
89665	6	399752	5	NULL	NULL	0	NULL	spermidine synthase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In Caenorhabditis elegans the polyamine synthetic pathway consists of three enzymes , ornithine decarboxylase ( ODC ) , S-adenosylmethionine decarboxylase ( AdoMetDC ) and spermidine synthase .
	manualset3
89666	1	399753	5	NULL	NULL	0	NULL	Cl ( - ) - depleted photosystem II	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In Cl ( - ) - depleted photosystem II , the inhibition occurred after formation of the S3 state in about half of the centers and probably after S2TyrZ + formation in the remaining centers .
	manualset3
89667	2	399753	5	NULL	NULL	0	NULL	inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In Cl ( - ) - depleted photosystem II , the inhibition occurred after formation of the S3 state in about half of the centers and probably after S2TyrZ + formation in the remaining centers .
	manualset3
89668	3	399753	5	NULL	NULL	0	NULL	formation of the S3 state	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In Cl ( - ) - depleted photosystem II , the inhibition occurred after formation of the S3 state in about half of the centers and probably after S2TyrZ + formation in the remaining centers .
	manualset3
89673	4	399753	5	NULL	NULL	0	NULL	centers	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In Cl ( - ) - depleted photosystem II , the inhibition occurred after formation of the S3 state in about half of the centers and probably after S2TyrZ + formation in the remaining centers .
	manualset3
89674	5	399753	5	NULL	NULL	0	NULL	S2TyrZ + formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In Cl ( - ) - depleted photosystem II , the inhibition occurred after formation of the S3 state in about half of the centers and probably after S2TyrZ + formation in the remaining centers .
	manualset3
89676	6	399753	5	NULL	NULL	0	NULL	centers	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In Cl ( - ) - depleted photosystem II , the inhibition occurred after formation of the S3 state in about half of the centers and probably after S2TyrZ + formation in the remaining centers .
	manualset3
89677	1	399754	5	NULL	NULL	0	NULL	DOCA-salt rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In DOCA-salt rats , tempol ( 30 to 300 micromol/kg ) dose-dependently decreased RSNA , MAP , and HR .
	manualset3
89678	2	399754	5	NULL	NULL	0	NULL	tempol ( 30 to 300 micromol/kg ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In DOCA-salt rats , tempol ( 30 to 300 micromol/kg ) dose-dependently decreased RSNA , MAP , and HR .
	manualset3
89679	3	399754	5	NULL	NULL	0	NULL	RSNA	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In DOCA-salt rats , tempol ( 30 to 300 micromol/kg ) dose-dependently decreased RSNA , MAP , and HR .
	manualset3
89680	4	399754	5	NULL	NULL	0	NULL	MAP	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In DOCA-salt rats , tempol ( 30 to 300 micromol/kg ) dose-dependently decreased RSNA , MAP , and HR .
	manualset3
89681	5	399754	5	NULL	NULL	0	NULL	HR	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In DOCA-salt rats , tempol ( 30 to 300 micromol/kg ) dose-dependently decreased RSNA , MAP , and HR .
	manualset3
89846	1	399755	5	NULL	NULL	0	NULL	E-PR293 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In E-PR293 cells , the 50 % inhibitory concentration of the cytotoxic effects by nelfinavir and saquinavir were as low as nanomolar levels , almost equal to those found in the HIV-infection assay .
	manualset3
89847	2	399755	5	NULL	NULL	0	NULL	50 % inhibitory concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In E-PR293 cells , the 50 % inhibitory concentration of the cytotoxic effects by nelfinavir and saquinavir were as low as nanomolar levels , almost equal to those found in the HIV-infection assay .
	manualset3
89848	3	399755	5	NULL	NULL	0	NULL	cytotoxic effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In E-PR293 cells , the 50 % inhibitory concentration of the cytotoxic effects by nelfinavir and saquinavir were as low as nanomolar levels , almost equal to those found in the HIV-infection assay .
	manualset3
89849	4	399755	5	NULL	NULL	0	NULL	nelfinavir	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In E-PR293 cells , the 50 % inhibitory concentration of the cytotoxic effects by nelfinavir and saquinavir were as low as nanomolar levels , almost equal to those found in the HIV-infection assay .
	manualset3
89850	5	399755	5	NULL	NULL	0	NULL	saquinavir	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In E-PR293 cells , the 50 % inhibitory concentration of the cytotoxic effects by nelfinavir and saquinavir were as low as nanomolar levels , almost equal to those found in the HIV-infection assay .
	manualset3
89851	6	399755	5	NULL	NULL	0	NULL	nanomolar levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In E-PR293 cells , the 50 % inhibitory concentration of the cytotoxic effects by nelfinavir and saquinavir were as low as nanomolar levels , almost equal to those found in the HIV-infection assay .
	manualset3
89852	7	399755	5	NULL	NULL	0	NULL	HIV-infection assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In E-PR293 cells , the 50 % inhibitory concentration of the cytotoxic effects by nelfinavir and saquinavir were as low as nanomolar levels , almost equal to those found in the HIV-infection assay .
	manualset3
89853	1	399756	5	NULL	NULL	0	NULL	Europe	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In Europe more than 80 % of gallbladder stones are cholesterol stones .
	manualset3
89854	2	399756	5	NULL	NULL	0	NULL	80 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In Europe more than 80 % of gallbladder stones are cholesterol stones .
	manualset3
89855	3	399756	5	NULL	NULL	0	NULL	gallbladder stones	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In Europe more than 80 % of gallbladder stones are cholesterol stones .
	manualset3
89856	4	399756	5	NULL	NULL	0	NULL	cholesterol stones	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In Europe more than 80 % of gallbladder stones are cholesterol stones .
	manualset3
89857	1	399757	5	NULL	NULL	0	NULL	Experiment 1	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In Experiment 1 , tilmicosin was given by subcutaneous injection ( 15 mg/kg ) twice , 48 hours apart , to four calves ; four control calves received no treatment .
	manualset3
89858	2	399757	5	NULL	NULL	0	NULL	tilmicosin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In Experiment 1 , tilmicosin was given by subcutaneous injection ( 15 mg/kg ) twice , 48 hours apart , to four calves ; four control calves received no treatment .
	manualset3
89859	3	399757	5	NULL	NULL	0	NULL	subcutaneous injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In Experiment 1 , tilmicosin was given by subcutaneous injection ( 15 mg/kg ) twice , 48 hours apart , to four calves ; four control calves received no treatment .
	manualset3
89860	4	399757	5	NULL	NULL	0	NULL	15 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In Experiment 1 , tilmicosin was given by subcutaneous injection ( 15 mg/kg ) twice , 48 hours apart , to four calves ; four control calves received no treatment .
	manualset3
89861	5	399757	5	NULL	NULL	0	NULL	48 hours apart	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In Experiment 1 , tilmicosin was given by subcutaneous injection ( 15 mg/kg ) twice , 48 hours apart , to four calves ; four control calves received no treatment .
	manualset3
89862	6	399757	5	NULL	NULL	0	NULL	four calves	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In Experiment 1 , tilmicosin was given by subcutaneous injection ( 15 mg/kg ) twice , 48 hours apart , to four calves ; four control calves received no treatment .
	manualset3
89863	7	399757	5	NULL	NULL	0	NULL	four control calves	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In Experiment 1 , tilmicosin was given by subcutaneous injection ( 15 mg/kg ) twice , 48 hours apart , to four calves ; four control calves received no treatment .
	manualset3
89864	8	399757	5	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In Experiment 1 , tilmicosin was given by subcutaneous injection ( 15 mg/kg ) twice , 48 hours apart , to four calves ; four control calves received no treatment .
	manualset3
89865	1	399758	5	NULL	NULL	0	NULL	Experiment 2	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In Experiment 2 , lizards from each habitat were either maintained under the conditions of Experiment 1 , or under extremely low relative humidity .
	manualset3
89866	2	399758	5	NULL	NULL	0	NULL	lizards	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In Experiment 2 , lizards from each habitat were either maintained under the conditions of Experiment 1 , or under extremely low relative humidity .
	manualset3
89867	3	399758	5	NULL	NULL	0	NULL	habitat	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In Experiment 2 , lizards from each habitat were either maintained under the conditions of Experiment 1 , or under extremely low relative humidity .
	manualset3
89868	4	399758	5	NULL	NULL	NULL	NULL	conditions of Experiment 1	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In Experiment 2 , lizards from each habitat were either maintained under the conditions of Experiment 1 , or under extremely low relative humidity .
	manualset3
89869	5	399758	5	NULL	NULL	0	NULL	extremely low relative humidity	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In Experiment 2 , lizards from each habitat were either maintained under the conditions of Experiment 1 , or under extremely low relative humidity .
	manualset3
89870	1	399759	5	NULL	NULL	0	NULL	Two cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Two cases of lymphomatous papillary cystadenoma ) .
	manualset3
89871	2	399759	5	NULL	NULL	0	NULL	lymphomatous papillary cystadenoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Two cases of lymphomatous papillary cystadenoma ) .
	manualset3
89872	1	399760	5	NULL	NULL	0	NULL	February 2000	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	In February 2000 , Wyeth Europe received clearancefor etanercept in 15 EU countries by the EMEA for the treatment of active arthritis in adults when the response to DMARDs has been inadequate ( 354844 ) .
	manualset3
89873	2	399760	5	NULL	NULL	0	NULL	Wyeth Europe	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In February 2000 , Wyeth Europe received clearancefor etanercept in 15 EU countries by the EMEA for the treatment of active arthritis in adults when the response to DMARDs has been inadequate ( 354844 ) .
	manualset3
89874	3	399760	5	NULL	NULL	0	NULL	clearance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In February 2000 , Wyeth Europe received clearancefor etanercept in 15 EU countries by the EMEA for the treatment of active arthritis in adults when the response to DMARDs has been inadequate ( 354844 ) .
	manualset3
89875	4	399760	5	NULL	NULL	0	NULL	etanercept	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In February 2000 , Wyeth Europe received clearancefor etanercept in 15 EU countries by the EMEA for the treatment of active arthritis in adults when the response to DMARDs has been inadequate ( 354844 ) .
	manualset3
89876	5	399760	5	NULL	NULL	0	NULL	15 EU countries	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In February 2000 , Wyeth Europe received clearancefor etanercept in 15 EU countries by the EMEA for the treatment of active arthritis in adults when the response to DMARDs has been inadequate ( 354844 ) .
	manualset3
89877	6	399760	5	NULL	NULL	NULL	NULL	EMEA	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In February 2000 , Wyeth Europe received clearancefor etanercept in 15 EU countries by the EMEA for the treatment of active arthritis in adults when the response to DMARDs has been inadequate ( 354844 ) .
	manualset3
89878	7	399760	5	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In February 2000 , Wyeth Europe received clearancefor etanercept in 15 EU countries by the EMEA for the treatment of active arthritis in adults when the response to DMARDs has been inadequate ( 354844 ) .
	manualset3
89879	8	399760	5	NULL	NULL	0	NULL	active arthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In February 2000 , Wyeth Europe received clearancefor etanercept in 15 EU countries by the EMEA for the treatment of active arthritis in adults when the response to DMARDs has been inadequate ( 354844 ) .
	manualset3
89880	9	399760	5	NULL	NULL	0	NULL	adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In February 2000 , Wyeth Europe received clearancefor etanercept in 15 EU countries by the EMEA for the treatment of active arthritis in adults when the response to DMARDs has been inadequate ( 354844 ) .
	manualset3
89881	10	399760	5	NULL	NULL	0	NULL	response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In February 2000 , Wyeth Europe received clearancefor etanercept in 15 EU countries by the EMEA for the treatment of active arthritis in adults when the response to DMARDs has been inadequate ( 354844 ) .
	manualset3
89882	11	399760	5	NULL	NULL	NULL	NULL	DMARDs	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In February 2000 , Wyeth Europe received clearancefor etanercept in 15 EU countries by the EMEA for the treatment of active arthritis in adults when the response to DMARDs has been inadequate ( 354844 ) .
	manualset3
89883	1	399761	5	NULL	NULL	0	NULL	H. neanderthalensis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In H. neanderthalensis and H. heidelbergensis , the root canals are wide , with small apical convergence .
	manualset3
89884	2	399761	5	NULL	NULL	0	NULL	H. heidelbergensis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In H. neanderthalensis and H. heidelbergensis , the root canals are wide , with small apical convergence .
	manualset3
89885	3	399761	5	NULL	NULL	0	NULL	root canals	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In H. neanderthalensis and H. heidelbergensis , the root canals are wide , with small apical convergence .
	manualset3
89886	4	399761	5	NULL	NULL	0	NULL	small apical convergence	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In H. neanderthalensis and H. heidelbergensis , the root canals are wide , with small apical convergence .
	manualset3
89887	1	399762	5	NULL	NULL	0	NULL	HEPES ( nominally HCO ( 3 ) ( - ) - free ) Tyrode solution	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In HEPES ( nominally HCO ( 3 ) ( - ) - free ) Tyrode solution , pH ( i ) recovery from induced intracellular acidosis could be blocked completely by 30 microM 3-methylsulfonyl-4-piperidinobenzoyl , guanidine hydrochloride ( HOE 694 ) , a specific NHE inhibitor , or by removing extracellular Na ( + ) .
	manualset3
89888	2	399762	5	NULL	NULL	NULL	NULL	pH ( i ) recovery	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In HEPES ( nominally HCO ( 3 ) ( - ) - free ) Tyrode solution , pH ( i ) recovery from induced intracellular acidosis could be blocked completely by 30 microM 3-methylsulfonyl-4-piperidinobenzoyl , guanidine hydrochloride ( HOE 694 ) , a specific NHE inhibitor , or by removing extracellular Na ( + ) .
	manualset3
89889	3	399762	5	NULL	NULL	0	NULL	induced intracellular acidosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In HEPES ( nominally HCO ( 3 ) ( - ) - free ) Tyrode solution , pH ( i ) recovery from induced intracellular acidosis could be blocked completely by 30 microM 3-methylsulfonyl-4-piperidinobenzoyl , guanidine hydrochloride ( HOE 694 ) , a specific NHE inhibitor , or by removing extracellular Na ( + ) .
	manualset3
89890	4	399762	5	NULL	NULL	NULL	NULL	30 microM 3-methylsulfonyl-4-piperidinobenzoyl	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In HEPES ( nominally HCO ( 3 ) ( - ) - free ) Tyrode solution , pH ( i ) recovery from induced intracellular acidosis could be blocked completely by 30 microM 3-methylsulfonyl-4-piperidinobenzoyl , guanidine hydrochloride ( HOE 694 ) , a specific NHE inhibitor , or by removing extracellular Na ( + ) .
	manualset3
89891	5	399762	5	NULL	NULL	NULL	NULL	guanidine hydrochloride ( HOE 694 )	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In HEPES ( nominally HCO ( 3 ) ( - ) - free ) Tyrode solution , pH ( i ) recovery from induced intracellular acidosis could be blocked completely by 30 microM 3-methylsulfonyl-4-piperidinobenzoyl , guanidine hydrochloride ( HOE 694 ) , a specific NHE inhibitor , or by removing extracellular Na ( + ) .
	manualset3
89892	6	399762	5	NULL	NULL	0	NULL	specific NHE inhibitor	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In HEPES ( nominally HCO ( 3 ) ( - ) - free ) Tyrode solution , pH ( i ) recovery from induced intracellular acidosis could be blocked completely by 30 microM 3-methylsulfonyl-4-piperidinobenzoyl , guanidine hydrochloride ( HOE 694 ) , a specific NHE inhibitor , or by removing extracellular Na ( + ) .
	manualset3
89893	7	399762	5	NULL	NULL	0	NULL	extracellular Na ( + )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In HEPES ( nominally HCO ( 3 ) ( - ) - free ) Tyrode solution , pH ( i ) recovery from induced intracellular acidosis could be blocked completely by 30 microM 3-methylsulfonyl-4-piperidinobenzoyl , guanidine hydrochloride ( HOE 694 ) , a specific NHE inhibitor , or by removing extracellular Na ( + ) .
	manualset3
89894	1	399763	5	NULL	NULL	0	NULL	India	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In India sterilization ( tubal ligation , vasectomy ) is the most widely used and relatively successful methods .
	manualset3
89895	2	399763	5	NULL	NULL	0	NULL	sterilization ( tubal ligation , vasectomy )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In India sterilization ( tubal ligation , vasectomy ) is the most widely used and relatively successful methods .
	manualset3
89896	3	399763	5	NULL	NULL	0	NULL	relatively successful methods	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In India sterilization ( tubal ligation , vasectomy ) is the most widely used and relatively successful methods .
	manualset3
89897	1	399764	5	NULL	NULL	0	NULL	Japan	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In Japan stomach cancer remains the leading cause of cancer-related mortality .
	manualset3
89898	2	399764	5	NULL	NULL	0	NULL	stomach cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In Japan stomach cancer remains the leading cause of cancer-related mortality .
	manualset3
89899	3	399764	5	NULL	NULL	0	NULL	leading cause	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In Japan stomach cancer remains the leading cause of cancer-related mortality .
	manualset3
89900	4	399764	5	NULL	NULL	0	NULL	cancer-related mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In Japan stomach cancer remains the leading cause of cancer-related mortality .
	manualset3
89901	1	399765	5	NULL	NULL	0	NULL	LMCA disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In LMCA disease , there is usually also disease in other parts of the coronary arterial tree .
	manualset3
89902	2	399765	5	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In LMCA disease , there is usually also disease in other parts of the coronary arterial tree .
	manualset3
89903	3	399765	5	NULL	NULL	0	NULL	coronary arterial tree	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In LMCA disease , there is usually also disease in other parts of the coronary arterial tree .
	manualset3
89904	1	399766	5	NULL	NULL	0	NULL	Lck-deficient Th2 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In Lck-deficient Th2 cells , however , CD43 ligation led to IL-4 production and an increase in the expression of CD25 and CD69 antigens but , surprisingly , no proliferation .
	manualset3
89905	2	399766	5	NULL	NULL	0	NULL	CD43 ligation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In Lck-deficient Th2 cells , however , CD43 ligation led to IL-4 production and an increase in the expression of CD25 and CD69 antigens but , surprisingly , no proliferation .
	manualset3
89906	3	399766	5	NULL	NULL	0	NULL	IL-4 production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In Lck-deficient Th2 cells , however , CD43 ligation led to IL-4 production and an increase in the expression of CD25 and CD69 antigens but , surprisingly , no proliferation .
	manualset3
89907	4	399766	5	NULL	NULL	0	NULL	expression of CD25 and CD69 antigens	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In Lck-deficient Th2 cells , however , CD43 ligation led to IL-4 production and an increase in the expression of CD25 and CD69 antigens but , surprisingly , no proliferation .
	manualset3
89908	5	399766	5	NULL	NULL	0	NULL	proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In Lck-deficient Th2 cells , however , CD43 ligation led to IL-4 production and an increase in the expression of CD25 and CD69 antigens but , surprisingly , no proliferation .
	manualset3
89909	1	399767	5	NULL	NULL	0	NULL	Model 2	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In Model 2 , the lifestyle and antisocial traits of psychopathy were assumed to lead to a lifestyle that increases the risk of traumatic exposure and subsequent posttraumatic stress .
	manualset3
89910	2	399767	5	NULL	NULL	0	NULL	lifestyle	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In Model 2 , the lifestyle and antisocial traits of psychopathy were assumed to lead to a lifestyle that increases the risk of traumatic exposure and subsequent posttraumatic stress .
	manualset3
89911	3	399767	5	NULL	NULL	0	NULL	antisocial traits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In Model 2 , the lifestyle and antisocial traits of psychopathy were assumed to lead to a lifestyle that increases the risk of traumatic exposure and subsequent posttraumatic stress .
	manualset3
89912	4	399767	5	NULL	NULL	0	NULL	psychopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In Model 2 , the lifestyle and antisocial traits of psychopathy were assumed to lead to a lifestyle that increases the risk of traumatic exposure and subsequent posttraumatic stress .
	manualset3
89913	5	399767	5	NULL	NULL	0	NULL	lifestyle	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In Model 2 , the lifestyle and antisocial traits of psychopathy were assumed to lead to a lifestyle that increases the risk of traumatic exposure and subsequent posttraumatic stress .
	manualset3
89914	6	399767	5	NULL	NULL	0	NULL	risk of traumatic exposure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In Model 2 , the lifestyle and antisocial traits of psychopathy were assumed to lead to a lifestyle that increases the risk of traumatic exposure and subsequent posttraumatic stress .
	manualset3
89915	7	399767	5	NULL	NULL	0	NULL	subsequent posttraumatic stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In Model 2 , the lifestyle and antisocial traits of psychopathy were assumed to lead to a lifestyle that increases the risk of traumatic exposure and subsequent posttraumatic stress .
	manualset3
89916	1	399768	5	NULL	NULL	0	NULL	NOD mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In NOD mice , disease begins earlier , affects 100 % of the animals , does not require boosting and leads to florid infiltrates circumscribed to lateral and dorsal prostatic lobes .
	manualset3
89917	2	399768	5	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In NOD mice , disease begins earlier , affects 100 % of the animals , does not require boosting and leads to florid infiltrates circumscribed to lateral and dorsal prostatic lobes .
	manualset3
89918	3	399768	5	NULL	NULL	0	NULL	100 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In NOD mice , disease begins earlier , affects 100 % of the animals , does not require boosting and leads to florid infiltrates circumscribed to lateral and dorsal prostatic lobes .
	manualset3
89919	4	399768	5	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In NOD mice , disease begins earlier , affects 100 % of the animals , does not require boosting and leads to florid infiltrates circumscribed to lateral and dorsal prostatic lobes .
	manualset3
89920	5	399768	5	NULL	NULL	NULL	NULL	florid infiltrate	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In NOD mice , disease begins earlier , affects 100 % of the animals , does not require boosting and leads to florid infiltrates circumscribed to lateral and dorsal prostatic lobes .
	manualset3
91213	6	399768	5	NULL	NULL	0	NULL	lateral and dorsal prostatic lobes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In NOD mice , disease begins earlier , affects 100 % of the animals , does not require boosting and leads to florid infiltrates circumscribed to lateral and dorsal prostatic lobes .
	manualset3
89921	1	399769	5	NULL	NULL	0	NULL	New York	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In New York the main reason for hospitalization is harmful behavior , while in London it is psychiatric symptoms .
	manualset3
89922	2	399769	5	NULL	NULL	0	NULL	hospitalization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In New York the main reason for hospitalization is harmful behavior , while in London it is psychiatric symptoms .
	manualset3
89923	3	399769	5	NULL	NULL	0	NULL	harmful behavior	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In New York the main reason for hospitalization is harmful behavior , while in London it is psychiatric symptoms .
	manualset3
89924	4	399769	5	NULL	NULL	0	NULL	London	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In New York the main reason for hospitalization is harmful behavior , while in London it is psychiatric symptoms .
	manualset3
89925	5	399769	5	NULL	NULL	0	NULL	psychiatric symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In New York the main reason for hospitalization is harmful behavior , while in London it is psychiatric symptoms .
	manualset3
89926	1	399770	5	NULL	NULL	NULL	NULL	Two strains of genetically hypertensive rats , LH and SRH	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Two strains of genetically hypertensive rats , LH and SRH , have distinct profiles of postnatal expression of tropoelastin and type III collagen in the aortic wall ) .
	manualset3
89927	2	399770	5	NULL	NULL	NULL	NULL	distinct profiles	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Two strains of genetically hypertensive rats , LH and SRH , have distinct profiles of postnatal expression of tropoelastin and type III collagen in the aortic wall ) .
	manualset3
89928	3	399770	5	NULL	NULL	0	NULL	postnatal expression of tropoelastin	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Two strains of genetically hypertensive rats , LH and SRH , have distinct profiles of postnatal expression of tropoelastin and type III collagen in the aortic wall ) .
	manualset3
89929	4	399770	5	NULL	NULL	0	NULL	postnatal expression of type III collagen	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Two strains of genetically hypertensive rats , LH and SRH , have distinct profiles of postnatal expression of tropoelastin and type III collagen in the aortic wall ) .
	manualset3
89930	5	399770	5	NULL	NULL	0	NULL	aortic wall	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Two strains of genetically hypertensive rats , LH and SRH , have distinct profiles of postnatal expression of tropoelastin and type III collagen in the aortic wall ) .
	manualset3
89931	1	399771	5	NULL	NULL	0	NULL	Northern blot analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In Northern blot analyses , VEGF induced Egr-1 mRNA levels in all tissues examined except lung and kidney , whereas EGF led to increased transcripts in all tissues except kidney .
	manualset3
90163	2	399771	5	NULL	NULL	0	NULL	VEGF induced Egr-1 mRNA levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In Northern blot analyses , VEGF induced Egr-1 mRNA levels in all tissues examined except lung and kidney , whereas EGF led to increased transcripts in all tissues except kidney .
	manualset3
90164	3	399771	5	NULL	NULL	0	NULL	tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In Northern blot analyses , VEGF induced Egr-1 mRNA levels in all tissues examined except lung and kidney , whereas EGF led to increased transcripts in all tissues except kidney .
	manualset3
90165	4	399771	5	NULL	NULL	0	NULL	lung tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In Northern blot analyses , VEGF induced Egr-1 mRNA levels in all tissues examined except lung and kidney , whereas EGF led to increased transcripts in all tissues except kidney .
	manualset3
90166	5	399771	5	NULL	NULL	0	NULL	kidney tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In Northern blot analyses , VEGF induced Egr-1 mRNA levels in all tissues examined except lung and kidney , whereas EGF led to increased transcripts in all tissues except kidney .
	manualset3
90167	6	399771	5	NULL	NULL	0	NULL	EGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In Northern blot analyses , VEGF induced Egr-1 mRNA levels in all tissues examined except lung and kidney , whereas EGF led to increased transcripts in all tissues except kidney .
	manualset3
90168	7	399771	5	NULL	NULL	0	NULL	increased transcripts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In Northern blot analyses , VEGF induced Egr-1 mRNA levels in all tissues examined except lung and kidney , whereas EGF led to increased transcripts in all tissues except kidney .
	manualset3
90169	8	399771	5	NULL	NULL	0	NULL	tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In Northern blot analyses , VEGF induced Egr-1 mRNA levels in all tissues examined except lung and kidney , whereas EGF led to increased transcripts in all tissues except kidney .
	manualset3
90170	9	399771	5	NULL	NULL	0	NULL	kidney tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In Northern blot analyses , VEGF induced Egr-1 mRNA levels in all tissues examined except lung and kidney , whereas EGF led to increased transcripts in all tissues except kidney .
	manualset3
90171	1	399772	5	NULL	NULL	0	NULL	P48 kittens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In P48 kittens , density and width of the plexus is reduced and axonal loop cells and the local axon cells have disappeared .
	manualset3
90172	2	399772	5	NULL	NULL	0	NULL	density	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In P48 kittens , density and width of the plexus is reduced and axonal loop cells and the local axon cells have disappeared .
	manualset3
90173	3	399772	5	NULL	NULL	0	NULL	width	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In P48 kittens , density and width of the plexus is reduced and axonal loop cells and the local axon cells have disappeared .
	manualset3
90174	4	399772	5	NULL	NULL	0	NULL	plexus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In P48 kittens , density and width of the plexus is reduced and axonal loop cells and the local axon cells have disappeared .
	manualset3
90175	5	399772	5	NULL	NULL	0	NULL	axonal loop cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In P48 kittens , density and width of the plexus is reduced and axonal loop cells and the local axon cells have disappeared .
	manualset3
90176	6	399772	5	NULL	NULL	0	NULL	local axon cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In P48 kittens , density and width of the plexus is reduced and axonal loop cells and the local axon cells have disappeared .
	manualset3
90177	1	399773	5	NULL	NULL	0	NULL	RFM / ( T6 X RFM ) F1 chimeras	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In RFM / ( T6 X RFM ) F1 chimeras , N-tropic murine leukemia virus can be detected as early as 3 days .
	manualset3
90178	2	399773	5	NULL	NULL	0	NULL	N-tropic murine leukemia virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In RFM / ( T6 X RFM ) F1 chimeras , N-tropic murine leukemia virus can be detected as early as 3 days .
	manualset3
90179	3	399773	5	NULL	NULL	0	NULL	3 days	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In RFM / ( T6 X RFM ) F1 chimeras , N-tropic murine leukemia virus can be detected as early as 3 days .
	manualset3
90180	1	399774	5	NULL	NULL	NULL	NULL	SIVmac155T3 infections	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In SIVmac155T3 infections , naive CD4 + T cells were dramatically depleted , but this population was spared by SIVmac239 , even in rapid progressors .
	manualset3
90181	2	399774	5	NULL	NULL	0	NULL	naive CD4 + T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In SIVmac155T3 infections , naive CD4 + T cells were dramatically depleted , but this population was spared by SIVmac239 , even in rapid progressors .
	manualset3
90182	3	399774	5	NULL	NULL	0	NULL	population	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In SIVmac155T3 infections , naive CD4 + T cells were dramatically depleted , but this population was spared by SIVmac239 , even in rapid progressors .
	manualset3
90183	4	399774	5	NULL	NULL	0	NULL	SIVmac239	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In SIVmac155T3 infections , naive CD4 + T cells were dramatically depleted , but this population was spared by SIVmac239 , even in rapid progressors .
	manualset3
90184	5	399774	5	NULL	NULL	0	NULL	progressors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In SIVmac155T3 infections , naive CD4 + T cells were dramatically depleted , but this population was spared by SIVmac239 , even in rapid progressors .
	manualset3
90185	1	399775	5	NULL	NULL	0	NULL	Streptococcus thermophilus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In Streptococcus thermophilus , a species belonging to the salivarius group , the oligopeptide transporter Ami is essential for comX expression under competence-inducing conditions .
	manualset3
90186	2	399775	5	NULL	NULL	0	NULL	species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In Streptococcus thermophilus , a species belonging to the salivarius group , the oligopeptide transporter Ami is essential for comX expression under competence-inducing conditions .
	manualset3
90187	3	399775	5	NULL	NULL	0	NULL	salivarius group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In Streptococcus thermophilus , a species belonging to the salivarius group , the oligopeptide transporter Ami is essential for comX expression under competence-inducing conditions .
	manualset3
90212	4	399775	5	NULL	NULL	0	NULL	oligopeptide transporter Ami	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In Streptococcus thermophilus , a species belonging to the salivarius group , the oligopeptide transporter Ami is essential for comX expression under competence-inducing conditions .
	manualset3
90213	5	399775	5	NULL	NULL	0	NULL	comX expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In Streptococcus thermophilus , a species belonging to the salivarius group , the oligopeptide transporter Ami is essential for comX expression under competence-inducing conditions .
	manualset3
90214	6	399775	5	NULL	NULL	0	NULL	competence-inducing conditions	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In Streptococcus thermophilus , a species belonging to the salivarius group , the oligopeptide transporter Ami is essential for comX expression under competence-inducing conditions .
	manualset3
90215	1	399776	5	NULL	NULL	0	NULL	Study 2	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In Study 2 , the authors found that although novices performed better on the target task when instructed by beginners , they did better on a different task within the same domain when instructed by experts .
	manualset3
90216	2	399776	5	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In Study 2 , the authors found that although novices performed better on the target task when instructed by beginners , they did better on a different task within the same domain when instructed by experts .
	manualset3
90217	3	399776	5	NULL	NULL	0	NULL	novices	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In Study 2 , the authors found that although novices performed better on the target task when instructed by beginners , they did better on a different task within the same domain when instructed by experts .
	manualset3
90218	4	399776	5	NULL	NULL	NULL	NULL	target task	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In Study 2 , the authors found that although novices performed better on the target task when instructed by beginners , they did better on a different task within the same domain when instructed by experts .
	manualset3
90219	5	399776	5	NULL	NULL	0	NULL	beginners	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In Study 2 , the authors found that although novices performed better on the target task when instructed by beginners , they did better on a different task within the same domain when instructed by experts .
	manualset3
90220	6	399776	5	NULL	NULL	NULL	NULL	task	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In Study 2 , the authors found that although novices performed better on the target task when instructed by beginners , they did better on a different task within the same domain when instructed by experts .
	manualset3
90221	7	399776	5	NULL	NULL	NULL	NULL	same domain	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In Study 2 , the authors found that although novices performed better on the target task when instructed by beginners , they did better on a different task within the same domain when instructed by experts .
	manualset3
90222	8	399776	5	NULL	NULL	0	NULL	experts	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In Study 2 , the authors found that although novices performed better on the target task when instructed by beginners , they did better on a different task within the same domain when instructed by experts .
	manualset3
90223	1	399777	5	NULL	NULL	0	NULL	Study 3	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In Study 3 , the authors show that counterattitudinal lying decreases dialectical complexity but increases elaborative complexity , implicating a strategic ( as opposed to a cognitive strain ) view of the lying-complexity relationship .
	manualset3
90224	2	399777	5	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In Study 3 , the authors show that counterattitudinal lying decreases dialectical complexity but increases elaborative complexity , implicating a strategic ( as opposed to a cognitive strain ) view of the lying-complexity relationship .
	manualset3
90243	3	399777	5	NULL	NULL	0	NULL	dialectical complexity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In Study 3 , the authors show that counterattitudinal lying decreases dialectical complexity but increases elaborative complexity , implicating a strategic ( as opposed to a cognitive strain ) view of the lying-complexity relationship .
	manualset3
90245	4	399777	5	NULL	NULL	0	NULL	elaborative complexity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In Study 3 , the authors show that counterattitudinal lying decreases dialectical complexity but increases elaborative complexity , implicating a strategic ( as opposed to a cognitive strain ) view of the lying-complexity relationship .
	manualset3
90247	5	399777	5	NULL	NULL	0	NULL	strategic ( as opposed to a cognitive strain ) view	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In Study 3 , the authors show that counterattitudinal lying decreases dialectical complexity but increases elaborative complexity , implicating a strategic ( as opposed to a cognitive strain ) view of the lying-complexity relationship .
	manualset3
90248	6	399777	5	NULL	NULL	0	NULL	lying-complexity relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In Study 3 , the authors show that counterattitudinal lying decreases dialectical complexity but increases elaborative complexity , implicating a strategic ( as opposed to a cognitive strain ) view of the lying-complexity relationship .
	manualset3
90252	1	399778	5	NULL	NULL	0	NULL	T lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In T lymphocytes , Nck plays a pivotal role in the T cell receptor ( TCR ) - induced reorganisation of the actin cytoskeleton and the formation of the immunological synapse .
	manualset3
90253	2	399778	5	NULL	NULL	0	NULL	Nck	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In T lymphocytes , Nck plays a pivotal role in the T cell receptor ( TCR ) - induced reorganisation of the actin cytoskeleton and the formation of the immunological synapse .
	manualset3
90254	3	399778	5	NULL	NULL	0	NULL	pivotal role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In T lymphocytes , Nck plays a pivotal role in the T cell receptor ( TCR ) - induced reorganisation of the actin cytoskeleton and the formation of the immunological synapse .
	manualset3
90255	4	399778	5	NULL	NULL	0	NULL	T cell receptor ( TCR ) - induced reorganisation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In T lymphocytes , Nck plays a pivotal role in the T cell receptor ( TCR ) - induced reorganisation of the actin cytoskeleton and the formation of the immunological synapse .
	manualset3
90256	5	399778	5	NULL	NULL	0	NULL	actin cytoskeleton	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In T lymphocytes , Nck plays a pivotal role in the T cell receptor ( TCR ) - induced reorganisation of the actin cytoskeleton and the formation of the immunological synapse .
	manualset3
90257	6	399778	5	NULL	NULL	NULL	NULL	formation of the immunological synapse	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In T lymphocytes , Nck plays a pivotal role in the T cell receptor ( TCR ) - induced reorganisation of the actin cytoskeleton and the formation of the immunological synapse .
	manualset3
90258	1	399779	5	NULL	NULL	0	NULL	TNA mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In TNA mice , NBQX activated mouse social behavior and ambivalent aggression , while CNQX and GYKI 52466 only increased anxiety .
	manualset3
90259	2	399779	5	NULL	NULL	0	NULL	NBQX activated mouse	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In TNA mice , NBQX activated mouse social behavior and ambivalent aggression , while CNQX and GYKI 52466 only increased anxiety .
	manualset3
90260	3	399779	5	NULL	NULL	0	NULL	social behavior	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In TNA mice , NBQX activated mouse social behavior and ambivalent aggression , while CNQX and GYKI 52466 only increased anxiety .
	manualset3
90261	4	399779	5	NULL	NULL	0	NULL	ambivalent aggression	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In TNA mice , NBQX activated mouse social behavior and ambivalent aggression , while CNQX and GYKI 52466 only increased anxiety .
	manualset3
90262	5	399779	5	NULL	NULL	0	NULL	CNQX	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In TNA mice , NBQX activated mouse social behavior and ambivalent aggression , while CNQX and GYKI 52466 only increased anxiety .
	manualset3
90263	6	399779	5	NULL	NULL	0	NULL	GYKI 52466	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In TNA mice , NBQX activated mouse social behavior and ambivalent aggression , while CNQX and GYKI 52466 only increased anxiety .
	manualset3
90264	7	399779	5	NULL	NULL	0	NULL	anxiety	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In TNA mice , NBQX activated mouse social behavior and ambivalent aggression , while CNQX and GYKI 52466 only increased anxiety .
	manualset3
90265	1	399780	5	NULL	NULL	0	NULL	Phase II study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a Phase II study , 82 patients with Philadelphia chromosome ( Ph ) - positive chronic myelogenous leukemia were treated with 3.5 million I.U. / d of recombinant interferon alpha-2c ( rIFN ) .
	manualset3
90267	2	399780	5	NULL	NULL	0	NULL	82 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In a Phase II study , 82 patients with Philadelphia chromosome ( Ph ) - positive chronic myelogenous leukemia were treated with 3.5 million I.U. / d of recombinant interferon alpha-2c ( rIFN ) .
	manualset3
90269	3	399780	5	NULL	NULL	0	NULL	Philadelphia chromosome ( Ph ) - positive chronic myelogenous leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In a Phase II study , 82 patients with Philadelphia chromosome ( Ph ) - positive chronic myelogenous leukemia were treated with 3.5 million I.U. / d of recombinant interferon alpha-2c ( rIFN ) .
	manualset3
90271	4	399780	5	NULL	NULL	0	NULL	3.5 million I.U. / d	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In a Phase II study , 82 patients with Philadelphia chromosome ( Ph ) - positive chronic myelogenous leukemia were treated with 3.5 million I.U. / d of recombinant interferon alpha-2c ( rIFN ) .
	manualset3
90277	5	399780	5	NULL	NULL	NULL	NULL	recombinant interferon alpha-2c ( rIFN )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a Phase II study , 82 patients with Philadelphia chromosome ( Ph ) - positive chronic myelogenous leukemia were treated with 3.5 million I.U. / d of recombinant interferon alpha-2c ( rIFN ) .
	manualset3
90294	1	399781	5	NULL	NULL	0	NULL	Streptococcus pneumoniae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In a Streptococcus pneumoniae lung infection induced by transtracheal challenge , the pathogen was not recovered after therapy with azithromycin ( ED50 7.9 mg/kg ) , while clarithromycin was not effective ( ED50 ) 100 mg/kg ) .
	manualset3
90295	2	399781	5	NULL	NULL	0	NULL	lung infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In a Streptococcus pneumoniae lung infection induced by transtracheal challenge , the pathogen was not recovered after therapy with azithromycin ( ED50 7.9 mg/kg ) , while clarithromycin was not effective ( ED50 ) 100 mg/kg ) .
	manualset3
90299	3	399781	5	NULL	NULL	0	NULL	transtracheal challenge	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In a Streptococcus pneumoniae lung infection induced by transtracheal challenge , the pathogen was not recovered after therapy with azithromycin ( ED50 7.9 mg/kg ) , while clarithromycin was not effective ( ED50 ) 100 mg/kg ) .
	manualset3
90300	4	399781	5	NULL	NULL	0	NULL	pathogen	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In a Streptococcus pneumoniae lung infection induced by transtracheal challenge , the pathogen was not recovered after therapy with azithromycin ( ED50 7.9 mg/kg ) , while clarithromycin was not effective ( ED50 ) 100 mg/kg ) .
	manualset3
90302	5	399781	5	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In a Streptococcus pneumoniae lung infection induced by transtracheal challenge , the pathogen was not recovered after therapy with azithromycin ( ED50 7.9 mg/kg ) , while clarithromycin was not effective ( ED50 ) 100 mg/kg ) .
	manualset3
90303	6	399781	5	NULL	NULL	0	NULL	azithromycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In a Streptococcus pneumoniae lung infection induced by transtracheal challenge , the pathogen was not recovered after therapy with azithromycin ( ED50 7.9 mg/kg ) , while clarithromycin was not effective ( ED50 ) 100 mg/kg ) .
	manualset3
90304	7	399781	5	NULL	NULL	0	NULL	ED50 7.9 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In a Streptococcus pneumoniae lung infection induced by transtracheal challenge , the pathogen was not recovered after therapy with azithromycin ( ED50 7.9 mg/kg ) , while clarithromycin was not effective ( ED50 ) 100 mg/kg ) .
	manualset3
90305	8	399781	5	NULL	NULL	0	NULL	clarithromycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In a Streptococcus pneumoniae lung infection induced by transtracheal challenge , the pathogen was not recovered after therapy with azithromycin ( ED50 7.9 mg/kg ) , while clarithromycin was not effective ( ED50 ) 100 mg/kg ) .
	manualset3
90306	9	399781	5	NULL	NULL	0	NULL	( ED50 ) 100 mg/kg )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In a Streptococcus pneumoniae lung infection induced by transtracheal challenge , the pathogen was not recovered after therapy with azithromycin ( ED50 7.9 mg/kg ) , while clarithromycin was not effective ( ED50 ) 100 mg/kg ) .
	manualset3
90307	1	399782	5	NULL	NULL	NULL	NULL	case report	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a case report , the Lazarus stress and coping framework is used to assess , intervene in , and evaluate care given to one family during an admission of a family member to the CCU .
	manualset3
90310	2	399782	5	NULL	NULL	0	NULL	Lazarus stress	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In a case report , the Lazarus stress and coping framework is used to assess , intervene in , and evaluate care given to one family during an admission of a family member to the CCU .
	manualset3
90314	3	399782	5	NULL	NULL	0	NULL	coping framework	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In a case report , the Lazarus stress and coping framework is used to assess , intervene in , and evaluate care given to one family during an admission of a family member to the CCU .
	manualset3
90316	4	399782	5	NULL	NULL	0	NULL	care	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In a case report , the Lazarus stress and coping framework is used to assess , intervene in , and evaluate care given to one family during an admission of a family member to the CCU .
	manualset3
90317	5	399782	5	NULL	NULL	0	NULL	family	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In a case report , the Lazarus stress and coping framework is used to assess , intervene in , and evaluate care given to one family during an admission of a family member to the CCU .
	manualset3
90319	6	399782	5	NULL	NULL	0	NULL	admission	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In a case report , the Lazarus stress and coping framework is used to assess , intervene in , and evaluate care given to one family during an admission of a family member to the CCU .
	manualset3
90320	7	399782	5	NULL	NULL	NULL	NULL	family member	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a case report , the Lazarus stress and coping framework is used to assess , intervene in , and evaluate care given to one family during an admission of a family member to the CCU .
	manualset3
90321	8	399782	5	NULL	NULL	0	NULL	CCU	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In a case report , the Lazarus stress and coping framework is used to assess , intervene in , and evaluate care given to one family during an admission of a family member to the CCU .
	manualset3
90326	1	399783	5	NULL	NULL	0	NULL	cohort of 43 women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In a cohort of 43 women with viable , singleton pregnancies , cervical dilatation greater than 4 cm , and absent labor between 20 and 27 weeks gestation , 22 women who underwent emergency cerclage within six hours of admission , were compared prospectively with 15 women who elected conservative bed rest treatment .
	manualset3
90327	2	399783	5	NULL	NULL	0	NULL	viable , singleton pregnancies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In a cohort of 43 women with viable , singleton pregnancies , cervical dilatation greater than 4 cm , and absent labor between 20 and 27 weeks gestation , 22 women who underwent emergency cerclage within six hours of admission , were compared prospectively with 15 women who elected conservative bed rest treatment .
	manualset3
90329	3	399783	5	NULL	NULL	0	NULL	cervical dilatation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In a cohort of 43 women with viable , singleton pregnancies , cervical dilatation greater than 4 cm , and absent labor between 20 and 27 weeks gestation , 22 women who underwent emergency cerclage within six hours of admission , were compared prospectively with 15 women who elected conservative bed rest treatment .
	manualset3
90330	4	399783	5	NULL	NULL	0	NULL	4 cm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In a cohort of 43 women with viable , singleton pregnancies , cervical dilatation greater than 4 cm , and absent labor between 20 and 27 weeks gestation , 22 women who underwent emergency cerclage within six hours of admission , were compared prospectively with 15 women who elected conservative bed rest treatment .
	manualset3
90331	5	399783	5	NULL	NULL	0	NULL	absent labor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In a cohort of 43 women with viable , singleton pregnancies , cervical dilatation greater than 4 cm , and absent labor between 20 and 27 weeks gestation , 22 women who underwent emergency cerclage within six hours of admission , were compared prospectively with 15 women who elected conservative bed rest treatment .
	manualset3
90333	6	399783	5	NULL	NULL	0	NULL	between 20 and 27 weeks gestation	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In a cohort of 43 women with viable , singleton pregnancies , cervical dilatation greater than 4 cm , and absent labor between 20 and 27 weeks gestation , 22 women who underwent emergency cerclage within six hours of admission , were compared prospectively with 15 women who elected conservative bed rest treatment .
	manualset3
90335	7	399783	5	NULL	NULL	0	NULL	22 women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In a cohort of 43 women with viable , singleton pregnancies , cervical dilatation greater than 4 cm , and absent labor between 20 and 27 weeks gestation , 22 women who underwent emergency cerclage within six hours of admission , were compared prospectively with 15 women who elected conservative bed rest treatment .
	manualset3
90338	8	399783	5	NULL	NULL	0	NULL	emergency cerclage	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In a cohort of 43 women with viable , singleton pregnancies , cervical dilatation greater than 4 cm , and absent labor between 20 and 27 weeks gestation , 22 women who underwent emergency cerclage within six hours of admission , were compared prospectively with 15 women who elected conservative bed rest treatment .
	manualset3
90340	9	399783	5	NULL	NULL	0	NULL	within six hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In a cohort of 43 women with viable , singleton pregnancies , cervical dilatation greater than 4 cm , and absent labor between 20 and 27 weeks gestation , 22 women who underwent emergency cerclage within six hours of admission , were compared prospectively with 15 women who elected conservative bed rest treatment .
	manualset3
90341	10	399783	5	NULL	NULL	0	NULL	admission	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In a cohort of 43 women with viable , singleton pregnancies , cervical dilatation greater than 4 cm , and absent labor between 20 and 27 weeks gestation , 22 women who underwent emergency cerclage within six hours of admission , were compared prospectively with 15 women who elected conservative bed rest treatment .
	manualset3
90343	11	399783	5	NULL	NULL	0	NULL	15 women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In a cohort of 43 women with viable , singleton pregnancies , cervical dilatation greater than 4 cm , and absent labor between 20 and 27 weeks gestation , 22 women who underwent emergency cerclage within six hours of admission , were compared prospectively with 15 women who elected conservative bed rest treatment .
	manualset3
90344	12	399783	5	NULL	NULL	0	NULL	conservative bed rest treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In a cohort of 43 women with viable , singleton pregnancies , cervical dilatation greater than 4 cm , and absent labor between 20 and 27 weeks gestation , 22 women who underwent emergency cerclage within six hours of admission , were compared prospectively with 15 women who elected conservative bed rest treatment .
	manualset3
90352	1	399784	5	NULL	NULL	0	NULL	cuticular bleeding time study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a cuticular bleeding time study , these animals also had only a partial correction , but in an FeCl3 carotid artery , thrombosis assay correction was equivalent to a 50 % to 100 % level .
	manualset3
90353	2	399784	5	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In a cuticular bleeding time study , these animals also had only a partial correction , but in an FeCl3 carotid artery , thrombosis assay correction was equivalent to a 50 % to 100 % level .
	manualset3
90354	3	399784	5	NULL	NULL	NULL	NULL	partial correction	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a cuticular bleeding time study , these animals also had only a partial correction , but in an FeCl3 carotid artery , thrombosis assay correction was equivalent to a 50 % to 100 % level .
	manualset3
90355	4	399784	5	NULL	NULL	0	NULL	FeCl3 carotid artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In a cuticular bleeding time study , these animals also had only a partial correction , but in an FeCl3 carotid artery , thrombosis assay correction was equivalent to a 50 % to 100 % level .
	manualset3
90387	5	399784	5	NULL	NULL	NULL	NULL	thrombosis assay correction	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a cuticular bleeding time study , these animals also had only a partial correction , but in an FeCl3 carotid artery , thrombosis assay correction was equivalent to a 50 % to 100 % level .
	manualset3
90388	6	399784	5	NULL	NULL	0	NULL	50 % to 100 % level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a cuticular bleeding time study , these animals also had only a partial correction , but in an FeCl3 carotid artery , thrombosis assay correction was equivalent to a 50 % to 100 % level .
	manualset3
90396	1	399785	5	NULL	NULL	0	NULL	Anti-glioma activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Anti-glioma activity of treatment by bone marrow stromal cells transfected with HSV-tk in the rat ) .
	manualset3
90397	2	399785	5	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Anti-glioma activity of treatment by bone marrow stromal cells transfected with HSV-tk in the rat ) .
	manualset3
90398	3	399785	5	NULL	NULL	0	NULL	bone marrow stromal cells transfected with HSV-tk	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	( Anti-glioma activity of treatment by bone marrow stromal cells transfected with HSV-tk in the rat ) .
	manualset3
90399	4	399785	5	NULL	NULL	0	NULL	rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Anti-glioma activity of treatment by bone marrow stromal cells transfected with HSV-tk in the rat ) .
	manualset3
90400	1	399786	5	NULL	NULL	NULL	NULL	Tyrosine kinase inhibitors	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Tyrosine kinase inhibitors in tumor therapy -- part 2 .
	manualset3
90401	2	399786	5	NULL	NULL	0	NULL	tumor therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Tyrosine kinase inhibitors in tumor therapy -- part 2 .
	manualset3
90402	1	399787	5	NULL	NULL	NULL	NULL	different model	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a different model , OT inhibited the development of tolerance to the stereotyped behavior-inducing effects of cocaine as well as cocaine intravenous self-administration in rats .
	manualset3
90403	2	399787	5	NULL	NULL	NULL	NULL	OT	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a different model , OT inhibited the development of tolerance to the stereotyped behavior-inducing effects of cocaine as well as cocaine intravenous self-administration in rats .
	manualset3
90404	3	399787	5	NULL	NULL	0	NULL	development of tolerance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In a different model , OT inhibited the development of tolerance to the stereotyped behavior-inducing effects of cocaine as well as cocaine intravenous self-administration in rats .
	manualset3
90406	4	399787	5	NULL	NULL	0	NULL	stereotyped behavior-inducing effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In a different model , OT inhibited the development of tolerance to the stereotyped behavior-inducing effects of cocaine as well as cocaine intravenous self-administration in rats .
	manualset3
90411	5	399787	5	NULL	NULL	0	NULL	cocaine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In a different model , OT inhibited the development of tolerance to the stereotyped behavior-inducing effects of cocaine as well as cocaine intravenous self-administration in rats .
	manualset3
90412	6	399787	5	NULL	NULL	0	NULL	cocaine intravenous self-administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In a different model , OT inhibited the development of tolerance to the stereotyped behavior-inducing effects of cocaine as well as cocaine intravenous self-administration in rats .
	manualset3
90413	7	399787	5	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In a different model , OT inhibited the development of tolerance to the stereotyped behavior-inducing effects of cocaine as well as cocaine intravenous self-administration in rats .
	manualset3
90416	1	399788	5	NULL	NULL	0	NULL	first study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a first study , the raw product was subjected to several combined high-pressure and temperature treatments for calculating a mathematical model by a response surface methodology .
	manualset3
90420	2	399788	5	NULL	NULL	0	NULL	raw product	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a first study , the raw product was subjected to several combined high-pressure and temperature treatments for calculating a mathematical model by a response surface methodology .
	manualset3
90422	3	399788	5	NULL	NULL	0	NULL	several combined high-pressure and temperature treatments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a first study , the raw product was subjected to several combined high-pressure and temperature treatments for calculating a mathematical model by a response surface methodology .
	manualset3
90423	4	399788	5	NULL	NULL	NULL	NULL	mathematical model	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a first study , the raw product was subjected to several combined high-pressure and temperature treatments for calculating a mathematical model by a response surface methodology .
	manualset3
90426	5	399788	5	NULL	NULL	0	NULL	response surface methodology	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a first study , the raw product was subjected to several combined high-pressure and temperature treatments for calculating a mathematical model by a response surface methodology .
	manualset3
90428	1	399789	5	NULL	NULL	0	NULL	fluconazole-resistant clinical isolate of C. albicans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In a fluconazole-resistant clinical isolate of C. albicans , a fungicidal effect was produced when fluconazole was combined with 6-NDA .
	manualset3
90429	2	399789	5	NULL	NULL	0	NULL	fungicidal effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In a fluconazole-resistant clinical isolate of C. albicans , a fungicidal effect was produced when fluconazole was combined with 6-NDA .
	manualset3
90430	3	399789	5	NULL	NULL	0	NULL	fluconazole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In a fluconazole-resistant clinical isolate of C. albicans , a fungicidal effect was produced when fluconazole was combined with 6-NDA .
	manualset3
90431	4	399789	5	NULL	NULL	0	NULL	6-NDA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In a fluconazole-resistant clinical isolate of C. albicans , a fungicidal effect was produced when fluconazole was combined with 6-NDA .
	manualset3
90432	1	399790	5	NULL	NULL	0	NULL	forward-genetic screen	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a forward-genetic screen , we uncovered a new component of the circadian output pathway , which we have termed dyschronic ( dysc ) .
	manualset3
90433	2	399790	5	NULL	NULL	0	NULL	new component	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a forward-genetic screen , we uncovered a new component of the circadian output pathway , which we have termed dyschronic ( dysc ) .
	manualset3
90434	3	399790	5	NULL	NULL	0	NULL	circadian output pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In a forward-genetic screen , we uncovered a new component of the circadian output pathway , which we have termed dyschronic ( dysc ) .
	manualset3
90435	4	399790	5	NULL	NULL	0	NULL	dyschronic ( dysc )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In a forward-genetic screen , we uncovered a new component of the circadian output pathway , which we have termed dyschronic ( dysc ) .
	manualset3
90436	1	399791	5	NULL	NULL	0	NULL	fourth group	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a fourth group , AdCBS and AdLDLr were co-administered .
	manualset3
90437	2	399791	5	NULL	NULL	NULL	NULL	AdCBS	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a fourth group , AdCBS and AdLDLr were co-administered .
	manualset3
90438	3	399791	5	NULL	NULL	0	NULL	AdLDLr	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In a fourth group , AdCBS and AdLDLr were co-administered .
	manualset3
90439	1	399792	5	NULL	NULL	0	NULL	matched-cohort study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a matched-cohort study in which ICU patients with serologic evidence of Mimivirus pneumonia were matched to ICU patients remaining seronegative for Mimivirus , positive serology was associated with an increased duration of both mechanical ventilation and ICU stay .
	manualset3
90440	2	399792	5	NULL	NULL	0	NULL	ICU patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In a matched-cohort study in which ICU patients with serologic evidence of Mimivirus pneumonia were matched to ICU patients remaining seronegative for Mimivirus , positive serology was associated with an increased duration of both mechanical ventilation and ICU stay .
	manualset3
90441	3	399792	5	NULL	NULL	0	NULL	serologic evidence	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a matched-cohort study in which ICU patients with serologic evidence of Mimivirus pneumonia were matched to ICU patients remaining seronegative for Mimivirus , positive serology was associated with an increased duration of both mechanical ventilation and ICU stay .
	manualset3
90442	4	399792	5	NULL	NULL	0	NULL	Mimivirus pneumonia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In a matched-cohort study in which ICU patients with serologic evidence of Mimivirus pneumonia were matched to ICU patients remaining seronegative for Mimivirus , positive serology was associated with an increased duration of both mechanical ventilation and ICU stay .
	manualset3
90443	5	399792	5	NULL	NULL	0	NULL	ICU patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In a matched-cohort study in which ICU patients with serologic evidence of Mimivirus pneumonia were matched to ICU patients remaining seronegative for Mimivirus , positive serology was associated with an increased duration of both mechanical ventilation and ICU stay .
	manualset3
90444	6	399792	5	NULL	NULL	0	NULL	Mimivirus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In a matched-cohort study in which ICU patients with serologic evidence of Mimivirus pneumonia were matched to ICU patients remaining seronegative for Mimivirus , positive serology was associated with an increased duration of both mechanical ventilation and ICU stay .
	manualset3
90445	7	399792	5	NULL	NULL	0	NULL	positive serology	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a matched-cohort study in which ICU patients with serologic evidence of Mimivirus pneumonia were matched to ICU patients remaining seronegative for Mimivirus , positive serology was associated with an increased duration of both mechanical ventilation and ICU stay .
	manualset3
90446	8	399792	5	NULL	NULL	0	NULL	increased duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In a matched-cohort study in which ICU patients with serologic evidence of Mimivirus pneumonia were matched to ICU patients remaining seronegative for Mimivirus , positive serology was associated with an increased duration of both mechanical ventilation and ICU stay .
	manualset3
90447	9	399792	5	NULL	NULL	0	NULL	mechanical ventilation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In a matched-cohort study in which ICU patients with serologic evidence of Mimivirus pneumonia were matched to ICU patients remaining seronegative for Mimivirus , positive serology was associated with an increased duration of both mechanical ventilation and ICU stay .
	manualset3
90448	10	399792	5	NULL	NULL	0	NULL	ICU stay	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In a matched-cohort study in which ICU patients with serologic evidence of Mimivirus pneumonia were matched to ICU patients remaining seronegative for Mimivirus , positive serology was associated with an increased duration of both mechanical ventilation and ICU stay .
	manualset3
90449	1	399793	5	NULL	NULL	0	NULL	 middle cerebral artery stroke model	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In a middle cerebral artery stroke model in the cat , we found a significant correlation between an edema index based on MRI and a sensitive metabolic index of ischemia , the in vivo oxidation status of mitochondrial cytochrome aa3 determined by near-infrared reflectance spectrophotometry ( r = -0.70 , alpha = 0.001 ) .
	manualset3
90450	2	399793	5	NULL	NULL	0	NULL	cat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In a middle cerebral artery stroke model in the cat , we found a significant correlation between an edema index based on MRI and a sensitive metabolic index of ischemia , the in vivo oxidation status of mitochondrial cytochrome aa3 determined by near-infrared reflectance spectrophotometry ( r = -0.70 , alpha = 0.001 ) .
	manualset3
90451	3	399793	5	NULL	NULL	0	NULL	significant correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In a middle cerebral artery stroke model in the cat , we found a significant correlation between an edema index based on MRI and a sensitive metabolic index of ischemia , the in vivo oxidation status of mitochondrial cytochrome aa3 determined by near-infrared reflectance spectrophotometry ( r = -0.70 , alpha = 0.001 ) .
	manualset3
90452	4	399793	5	NULL	NULL	0	NULL	edema index	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a middle cerebral artery stroke model in the cat , we found a significant correlation between an edema index based on MRI and a sensitive metabolic index of ischemia , the in vivo oxidation status of mitochondrial cytochrome aa3 determined by near-infrared reflectance spectrophotometry ( r = -0.70 , alpha = 0.001 ) .
	manualset3
90453	5	399793	5	NULL	NULL	0	NULL	MRI	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In a middle cerebral artery stroke model in the cat , we found a significant correlation between an edema index based on MRI and a sensitive metabolic index of ischemia , the in vivo oxidation status of mitochondrial cytochrome aa3 determined by near-infrared reflectance spectrophotometry ( r = -0.70 , alpha = 0.001 ) .
	manualset3
90454	6	399793	5	NULL	NULL	0	NULL	sensitive metabolic index	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a middle cerebral artery stroke model in the cat , we found a significant correlation between an edema index based on MRI and a sensitive metabolic index of ischemia , the in vivo oxidation status of mitochondrial cytochrome aa3 determined by near-infrared reflectance spectrophotometry ( r = -0.70 , alpha = 0.001 ) .
	manualset3
90455	7	399793	5	NULL	NULL	0	NULL	ischemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In a middle cerebral artery stroke model in the cat , we found a significant correlation between an edema index based on MRI and a sensitive metabolic index of ischemia , the in vivo oxidation status of mitochondrial cytochrome aa3 determined by near-infrared reflectance spectrophotometry ( r = -0.70 , alpha = 0.001 ) .
	manualset3
90456	8	399793	5	NULL	NULL	0	NULL	in vivo oxidation status	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In a middle cerebral artery stroke model in the cat , we found a significant correlation between an edema index based on MRI and a sensitive metabolic index of ischemia , the in vivo oxidation status of mitochondrial cytochrome aa3 determined by near-infrared reflectance spectrophotometry ( r = -0.70 , alpha = 0.001 ) .
	manualset3
90457	9	399793	5	NULL	NULL	0	NULL	mitochondrial cytochrome aa3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In a middle cerebral artery stroke model in the cat , we found a significant correlation between an edema index based on MRI and a sensitive metabolic index of ischemia , the in vivo oxidation status of mitochondrial cytochrome aa3 determined by near-infrared reflectance spectrophotometry ( r = -0.70 , alpha = 0.001 ) .
	manualset3
90458	10	399793	5	NULL	NULL	0	NULL	near-infrared reflectance spectrophotometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a middle cerebral artery stroke model in the cat , we found a significant correlation between an edema index based on MRI and a sensitive metabolic index of ischemia , the in vivo oxidation status of mitochondrial cytochrome aa3 determined by near-infrared reflectance spectrophotometry ( r = -0.70 , alpha = 0.001 ) .
	manualset3
90459	11	399793	5	NULL	NULL	0	NULL	r = -0.70 , alpha = 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In a middle cerebral artery stroke model in the cat , we found a significant correlation between an edema index based on MRI and a sensitive metabolic index of ischemia , the in vivo oxidation status of mitochondrial cytochrome aa3 determined by near-infrared reflectance spectrophotometry ( r = -0.70 , alpha = 0.001 ) .
	manualset3
90460	1	399794	5	NULL	NULL	0	NULL	UNILATERAL SURGICAL RECURRENT NERVE LESION	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( UNILATERAL SURGICAL RECURRENT NERVE LESION AS AN INDICATION FOR TRACHEOTOMY ) .
	manualset3
90461	2	399794	5	NULL	NULL	0	NULL	INDICATION	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( UNILATERAL SURGICAL RECURRENT NERVE LESION AS AN INDICATION FOR TRACHEOTOMY ) .
	manualset3
90462	3	399794	5	NULL	NULL	0	NULL	TRACHEOTOMY	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( UNILATERAL SURGICAL RECURRENT NERVE LESION AS AN INDICATION FOR TRACHEOTOMY ) .
	manualset3
90463	1	399795	5	NULL	NULL	0	NULL	mouse model	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In a mouse model it was recently confirmed that recombinant murine ( rm - ) APC decreases coagulation activation and improves survival in pneumococcal pneumonia ; however , APC did not impact on the inflammatory response .
	manualset3
90464	2	399795	5	NULL	NULL	0	NULL	recombinant murine ( rm - ) APC	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In a mouse model it was recently confirmed that recombinant murine ( rm - ) APC decreases coagulation activation and improves survival in pneumococcal pneumonia ; however , APC did not impact on the inflammatory response .
	manualset3
90465	3	399795	5	NULL	NULL	0	NULL	coagulation activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In a mouse model it was recently confirmed that recombinant murine ( rm - ) APC decreases coagulation activation and improves survival in pneumococcal pneumonia ; however , APC did not impact on the inflammatory response .
	manualset3
90466	4	399795	5	NULL	NULL	0	NULL	survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In a mouse model it was recently confirmed that recombinant murine ( rm - ) APC decreases coagulation activation and improves survival in pneumococcal pneumonia ; however , APC did not impact on the inflammatory response .
	manualset3
90467	5	399795	5	NULL	NULL	0	NULL	pneumococcal pneumonia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In a mouse model it was recently confirmed that recombinant murine ( rm - ) APC decreases coagulation activation and improves survival in pneumococcal pneumonia ; however , APC did not impact on the inflammatory response .
	manualset3
90468	6	399795	5	NULL	NULL	0	NULL	APC	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In a mouse model it was recently confirmed that recombinant murine ( rm - ) APC decreases coagulation activation and improves survival in pneumococcal pneumonia ; however , APC did not impact on the inflammatory response .
	manualset3
90469	7	399795	5	NULL	NULL	0	NULL	inflammatory response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In a mouse model it was recently confirmed that recombinant murine ( rm - ) APC decreases coagulation activation and improves survival in pneumococcal pneumonia ; however , APC did not impact on the inflammatory response .
	manualset3
90470	1	399796	5	NULL	NULL	NULL	NULL	multilevel model of the data	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a multilevel model of the data there was a highly significant ( p & lt ; 0.001 ) effect of month of sampling on the frequency of AFM ( 1 ) detection with summer months having the highest frequency ( ) 80 % ) and winter months the lowest frequency ( & lt ; 20 % ) of detection .
	manualset3
90471	3	399796	5	NULL	NULL	NULL	NULL	( p & lt ; 0.001 )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a multilevel model of the data there was a highly significant ( p & lt ; 0.001 ) effect of month of sampling on the frequency of AFM ( 1 ) detection with summer months having the highest frequency ( ) 80 % ) and winter months the lowest frequency ( & lt ; 20 % ) of detection .
	manualset3
90472	2	399796	5	NULL	NULL	NULL	NULL	highly significant effect	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a multilevel model of the data there was a highly significant ( p & lt ; 0.001 ) effect of month of sampling on the frequency of AFM ( 1 ) detection with summer months having the highest frequency ( ) 80 % ) and winter months the lowest frequency ( & lt ; 20 % ) of detection .
	manualset3
91083	4	399796	5	NULL	NULL	NULL	NULL	month	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a multilevel model of the data there was a highly significant ( p & lt ; 0.001 ) effect of month of sampling on the frequency of AFM ( 1 ) detection with summer months having the highest frequency ( ) 80 % ) and winter months the lowest frequency ( & lt ; 20 % ) of detection .
	manualset3
91084	6	399796	5	NULL	NULL	NULL	NULL	frequency	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a multilevel model of the data there was a highly significant ( p & lt ; 0.001 ) effect of month of sampling on the frequency of AFM ( 1 ) detection with summer months having the highest frequency ( ) 80 % ) and winter months the lowest frequency ( & lt ; 20 % ) of detection .
	manualset3
91085	7	399796	5	NULL	NULL	NULL	NULL	AFM	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a multilevel model of the data there was a highly significant ( p & lt ; 0.001 ) effect of month of sampling on the frequency of AFM ( 1 ) detection with summer months having the highest frequency ( ) 80 % ) and winter months the lowest frequency ( & lt ; 20 % ) of detection .
	manualset3
91086	9	399796	5	NULL	NULL	NULL	NULL	summer months	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a multilevel model of the data there was a highly significant ( p & lt ; 0.001 ) effect of month of sampling on the frequency of AFM ( 1 ) detection with summer months having the highest frequency ( ) 80 % ) and winter months the lowest frequency ( & lt ; 20 % ) of detection .
	manualset3
91087	10	399796	5	NULL	NULL	NULL	NULL	highest frequency	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a multilevel model of the data there was a highly significant ( p & lt ; 0.001 ) effect of month of sampling on the frequency of AFM ( 1 ) detection with summer months having the highest frequency ( ) 80 % ) and winter months the lowest frequency ( & lt ; 20 % ) of detection .
	manualset3
91088	12	399796	5	NULL	NULL	NULL	NULL	winter months	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a multilevel model of the data there was a highly significant ( p & lt ; 0.001 ) effect of month of sampling on the frequency of AFM ( 1 ) detection with summer months having the highest frequency ( ) 80 % ) and winter months the lowest frequency ( & lt ; 20 % ) of detection .
	manualset3
91089	13	399796	5	NULL	NULL	NULL	NULL	lowest frequency	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a multilevel model of the data there was a highly significant ( p & lt ; 0.001 ) effect of month of sampling on the frequency of AFM ( 1 ) detection with summer months having the highest frequency ( ) 80 % ) and winter months the lowest frequency ( & lt ; 20 % ) of detection .
	manualset3
91090	5	399796	5	NULL	NULL	0	NULL	sampling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a multilevel model of the data there was a highly significant ( p & lt ; 0.001 ) effect of month of sampling on the frequency of AFM ( 1 ) detection with summer months having the highest frequency ( ) 80 % ) and winter months the lowest frequency ( & lt ; 20 % ) of detection .
	manualset3
91091	8	399796	5	NULL	NULL	0	NULL	detection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In a multilevel model of the data there was a highly significant ( p & lt ; 0.001 ) effect of month of sampling on the frequency of AFM ( 1 ) detection with summer months having the highest frequency ( ) 80 % ) and winter months the lowest frequency ( & lt ; 20 % ) of detection .
	manualset3
91214	11	399796	5	NULL	NULL	0	NULL	80 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In a multilevel model of the data there was a highly significant ( p & lt ; 0.001 ) effect of month of sampling on the frequency of AFM ( 1 ) detection with summer months having the highest frequency ( ) 80 % ) and winter months the lowest frequency ( & lt ; 20 % ) of detection .
	manualset3
91215	14	399796	5	NULL	NULL	0	NULL	( & lt ; 20 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In a multilevel model of the data there was a highly significant ( p & lt ; 0.001 ) effect of month of sampling on the frequency of AFM ( 1 ) detection with summer months having the highest frequency ( ) 80 % ) and winter months the lowest frequency ( & lt ; 20 % ) of detection .
	manualset3
90616	1	399797	5	NULL	NULL	NULL	NULL	patient with Wolff-Parkinson-White syndrome	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a patient with Wolff-Parkinson-White syndrome , rapid atrial pacing up to rates of 140/min resulted in A-H prolongation ; increases in rate up to 200/min , however , failed to lengthen A-H further .
	manualset3
90617	2	399797	5	NULL	NULL	0	NULL	atrial pacing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In a patient with Wolff-Parkinson-White syndrome , rapid atrial pacing up to rates of 140/min resulted in A-H prolongation ; increases in rate up to 200/min , however , failed to lengthen A-H further .
	manualset3
90618	3	399797	5	NULL	NULL	0	NULL	rates of 140/min	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In a patient with Wolff-Parkinson-White syndrome , rapid atrial pacing up to rates of 140/min resulted in A-H prolongation ; increases in rate up to 200/min , however , failed to lengthen A-H further .
	manualset3
90619	4	399797	5	NULL	NULL	0	NULL	A-H prolongation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In a patient with Wolff-Parkinson-White syndrome , rapid atrial pacing up to rates of 140/min resulted in A-H prolongation ; increases in rate up to 200/min , however , failed to lengthen A-H further .
	manualset3
90620	5	399797	5	NULL	NULL	0	NULL	rate up to 200/min	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In a patient with Wolff-Parkinson-White syndrome , rapid atrial pacing up to rates of 140/min resulted in A-H prolongation ; increases in rate up to 200/min , however , failed to lengthen A-H further .
	manualset3
90621	6	399797	5	NULL	NULL	0	NULL	A-H	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In a patient with Wolff-Parkinson-White syndrome , rapid atrial pacing up to rates of 140/min resulted in A-H prolongation ; increases in rate up to 200/min , however , failed to lengthen A-H further .
	manualset3
90622	1	399798	5	NULL	NULL	NULL	NULL	dose-response study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a previous step a dose-response study of the behavioral effects of scopolamine , in doses of 0.05 , 0.1 , 0.4 and 0.8 mg/kg was carried out in ten cats .
	manualset3
90623	2	399798	5	NULL	NULL	0	NULL	behavioral effects	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous step a dose-response study of the behavioral effects of scopolamine , in doses of 0.05 , 0.1 , 0.4 and 0.8 mg/kg was carried out in ten cats .
	manualset3
90624	3	399798	5	NULL	NULL	0	NULL	scopolamine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous step a dose-response study of the behavioral effects of scopolamine , in doses of 0.05 , 0.1 , 0.4 and 0.8 mg/kg was carried out in ten cats .
	manualset3
90625	4	399798	5	NULL	NULL	0	NULL	doses of 0.05 , 0.1 , 0.4 and 0.8 mg/kg	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous step a dose-response study of the behavioral effects of scopolamine , in doses of 0.05 , 0.1 , 0.4 and 0.8 mg/kg was carried out in ten cats .
	manualset3
90626	5	399798	5	NULL	NULL	0	NULL	ten cats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous step a dose-response study of the behavioral effects of scopolamine , in doses of 0.05 , 0.1 , 0.4 and 0.8 mg/kg was carried out in ten cats .
	manualset3
90627	1	399799	5	NULL	NULL	0	NULL	 previous study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous study , we demonstrated that diethylstilbestrol ( DES ) , a non-steroidal estrogen , induces fish oocyte maturation via the membrane progestin receptor ( mPR ) .
	manualset3
90628	2	399799	5	NULL	NULL	0	NULL	diethylstilbestrol ( DES )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous study , we demonstrated that diethylstilbestrol ( DES ) , a non-steroidal estrogen , induces fish oocyte maturation via the membrane progestin receptor ( mPR ) .
	manualset3
90629	3	399799	5	NULL	NULL	0	NULL	non-steroidal estrogen	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous study , we demonstrated that diethylstilbestrol ( DES ) , a non-steroidal estrogen , induces fish oocyte maturation via the membrane progestin receptor ( mPR ) .
	manualset3
90630	4	399799	5	NULL	NULL	0	NULL	fish oocyte maturation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous study , we demonstrated that diethylstilbestrol ( DES ) , a non-steroidal estrogen , induces fish oocyte maturation via the membrane progestin receptor ( mPR ) .
	manualset3
90631	5	399799	5	NULL	NULL	0	NULL	membrane progestin receptor ( mPR )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous study , we demonstrated that diethylstilbestrol ( DES ) , a non-steroidal estrogen , induces fish oocyte maturation via the membrane progestin receptor ( mPR ) .
	manualset3
90632	1	399800	5	NULL	NULL	0	NULL	previous study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous study we reported that oligomerized T cell epitopes `` superactivated '' CD4 + T cells .
	manualset3
90633	2	399800	5	NULL	NULL	0	NULL	oligomerized T cell epitopes	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous study we reported that oligomerized T cell epitopes `` superactivated '' CD4 + T cells .
	manualset3
90634	3	399800	5	NULL	NULL	0	NULL	CD4 + T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous study we reported that oligomerized T cell epitopes `` superactivated '' CD4 + T cells .
	manualset3
90635	1	399801	5	NULL	NULL	0	NULL	 previous study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous study we showed that EGF receptor levels in rat granulosa cells were increased up to fourfold after 96 h of culture with human GH in the presence of FSH , and the present study has evaluated the action of EGF on these cells .
	manualset3
90636	2	399801	5	NULL	NULL	0	NULL	EGF receptor levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous study we showed that EGF receptor levels in rat granulosa cells were increased up to fourfold after 96 h of culture with human GH in the presence of FSH , and the present study has evaluated the action of EGF on these cells .
	manualset3
90637	3	399801	5	NULL	NULL	0	NULL	rat granulosa cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous study we showed that EGF receptor levels in rat granulosa cells were increased up to fourfold after 96 h of culture with human GH in the presence of FSH , and the present study has evaluated the action of EGF on these cells .
	manualset3
90638	4	399801	5	NULL	NULL	0	NULL	96 h of culture	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous study we showed that EGF receptor levels in rat granulosa cells were increased up to fourfold after 96 h of culture with human GH in the presence of FSH , and the present study has evaluated the action of EGF on these cells .
	manualset3
90639	5	399801	5	NULL	NULL	0	NULL	human GH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous study we showed that EGF receptor levels in rat granulosa cells were increased up to fourfold after 96 h of culture with human GH in the presence of FSH , and the present study has evaluated the action of EGF on these cells .
	manualset3
90640	6	399801	5	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous study we showed that EGF receptor levels in rat granulosa cells were increased up to fourfold after 96 h of culture with human GH in the presence of FSH , and the present study has evaluated the action of EGF on these cells .
	manualset3
90641	7	399801	5	NULL	NULL	0	NULL	FSH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous study we showed that EGF receptor levels in rat granulosa cells were increased up to fourfold after 96 h of culture with human GH in the presence of FSH , and the present study has evaluated the action of EGF on these cells .
	manualset3
90642	8	399801	5	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous study we showed that EGF receptor levels in rat granulosa cells were increased up to fourfold after 96 h of culture with human GH in the presence of FSH , and the present study has evaluated the action of EGF on these cells .
	manualset3
90643	9	399801	5	NULL	NULL	0	NULL	action of EGF	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous study we showed that EGF receptor levels in rat granulosa cells were increased up to fourfold after 96 h of culture with human GH in the presence of FSH , and the present study has evaluated the action of EGF on these cells .
	manualset3
90644	10	399801	5	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous study we showed that EGF receptor levels in rat granulosa cells were increased up to fourfold after 96 h of culture with human GH in the presence of FSH , and the present study has evaluated the action of EGF on these cells .
	manualset3
90645	1	399802	5	NULL	NULL	NULL	NULL	prospective epidemiological study data of 24	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a prospective epidemiological study data of 24 , 732 pregnancies were analyzed by computer programs for the incidence of congenital heart disease ( CHD ) and its relationship to various factors affecting pregnancy ( age and weight of mother , smoking , alcohol - , and coffee-consumption , usage of oral contraception ) .
	manualset3
90646	2	399802	5	NULL	NULL	NULL	NULL	732 pregnancies	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a prospective epidemiological study data of 24 , 732 pregnancies were analyzed by computer programs for the incidence of congenital heart disease ( CHD ) and its relationship to various factors affecting pregnancy ( age and weight of mother , smoking , alcohol - , and coffee-consumption , usage of oral contraception ) .
	manualset3
90647	3	399802	5	NULL	NULL	0	NULL	computer programs	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In a prospective epidemiological study data of 24 , 732 pregnancies were analyzed by computer programs for the incidence of congenital heart disease ( CHD ) and its relationship to various factors affecting pregnancy ( age and weight of mother , smoking , alcohol - , and coffee-consumption , usage of oral contraception ) .
	manualset3
90648	4	399802	5	NULL	NULL	0	NULL	incidence of congenital heart disease ( CHD )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In a prospective epidemiological study data of 24 , 732 pregnancies were analyzed by computer programs for the incidence of congenital heart disease ( CHD ) and its relationship to various factors affecting pregnancy ( age and weight of mother , smoking , alcohol - , and coffee-consumption , usage of oral contraception ) .
	manualset3
90649	5	399802	5	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In a prospective epidemiological study data of 24 , 732 pregnancies were analyzed by computer programs for the incidence of congenital heart disease ( CHD ) and its relationship to various factors affecting pregnancy ( age and weight of mother , smoking , alcohol - , and coffee-consumption , usage of oral contraception ) .
	manualset3
90650	6	399802	5	NULL	NULL	0	NULL	various factors affecting pregnancy	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In a prospective epidemiological study data of 24 , 732 pregnancies were analyzed by computer programs for the incidence of congenital heart disease ( CHD ) and its relationship to various factors affecting pregnancy ( age and weight of mother , smoking , alcohol - , and coffee-consumption , usage of oral contraception ) .
	manualset3
90651	7	399802	5	NULL	NULL	0	NULL	age and weight of mother	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In a prospective epidemiological study data of 24 , 732 pregnancies were analyzed by computer programs for the incidence of congenital heart disease ( CHD ) and its relationship to various factors affecting pregnancy ( age and weight of mother , smoking , alcohol - , and coffee-consumption , usage of oral contraception ) .
	manualset3
90652	8	399802	5	NULL	NULL	0	NULL	smoking	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In a prospective epidemiological study data of 24 , 732 pregnancies were analyzed by computer programs for the incidence of congenital heart disease ( CHD ) and its relationship to various factors affecting pregnancy ( age and weight of mother , smoking , alcohol - , and coffee-consumption , usage of oral contraception ) .
	manualset3
90653	9	399802	5	NULL	NULL	0	NULL	alcohol - , and coffee-consumption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In a prospective epidemiological study data of 24 , 732 pregnancies were analyzed by computer programs for the incidence of congenital heart disease ( CHD ) and its relationship to various factors affecting pregnancy ( age and weight of mother , smoking , alcohol - , and coffee-consumption , usage of oral contraception ) .
	manualset3
90654	10	399802	5	NULL	NULL	0	NULL	usage of oral contraception	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In a prospective epidemiological study data of 24 , 732 pregnancies were analyzed by computer programs for the incidence of congenital heart disease ( CHD ) and its relationship to various factors affecting pregnancy ( age and weight of mother , smoking , alcohol - , and coffee-consumption , usage of oral contraception ) .
	manualset3
90655	1	399803	5	NULL	NULL	0	NULL	prospective genetic association study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a prospective genetic association study we genotyped 542 patients with CSF culture proven community acquired bacterial meningitis and 376 matched controls for 2 functional single nucleotide polymorphisms in the 2-adrenoceptor gene ( ADRB2 ) .
	manualset3
90656	2	399803	5	NULL	NULL	0	NULL	542 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In a prospective genetic association study we genotyped 542 patients with CSF culture proven community acquired bacterial meningitis and 376 matched controls for 2 functional single nucleotide polymorphisms in the 2-adrenoceptor gene ( ADRB2 ) .
	manualset3
90657	3	399803	5	NULL	NULL	NULL	NULL	CSF culture proven community acquired bacterial meningitis	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a prospective genetic association study we genotyped 542 patients with CSF culture proven community acquired bacterial meningitis and 376 matched controls for 2 functional single nucleotide polymorphisms in the 2-adrenoceptor gene ( ADRB2 ) .
	manualset3
90658	4	399803	5	NULL	NULL	0	NULL	376	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In a prospective genetic association study we genotyped 542 patients with CSF culture proven community acquired bacterial meningitis and 376 matched controls for 2 functional single nucleotide polymorphisms in the 2-adrenoceptor gene ( ADRB2 ) .
	manualset3
90659	5	399803	5	NULL	NULL	0	NULL	controls	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In a prospective genetic association study we genotyped 542 patients with CSF culture proven community acquired bacterial meningitis and 376 matched controls for 2 functional single nucleotide polymorphisms in the 2-adrenoceptor gene ( ADRB2 ) .
	manualset3
90660	6	399803	5	NULL	NULL	NULL	NULL	2 functional single nucleotide polymorphisms	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a prospective genetic association study we genotyped 542 patients with CSF culture proven community acquired bacterial meningitis and 376 matched controls for 2 functional single nucleotide polymorphisms in the 2-adrenoceptor gene ( ADRB2 ) .
	manualset3
90661	7	399803	5	NULL	NULL	0	NULL	2-adrenoceptor gene ( ADRB2 )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In a prospective genetic association study we genotyped 542 patients with CSF culture proven community acquired bacterial meningitis and 376 matched controls for 2 functional single nucleotide polymorphisms in the 2-adrenoceptor gene ( ADRB2 ) .
	manualset3
90662	1	399804	5	NULL	NULL	0	NULL	prospective study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a prospective study from 1991-1998 plasma concentrations of alpha-Tocopherole ( VitE ) and Selenium ( Se ) were analyzed in 125 sheep and 32 goats with generalised motor disturbances or elevated plasma-activities of Creatine-Kinase ( CK ) .
	manualset3
90663	2	399804	5	NULL	NULL	0	NULL	1991-1998	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In a prospective study from 1991-1998 plasma concentrations of alpha-Tocopherole ( VitE ) and Selenium ( Se ) were analyzed in 125 sheep and 32 goats with generalised motor disturbances or elevated plasma-activities of Creatine-Kinase ( CK ) .
	manualset3
90664	3	399804	5	NULL	NULL	0	NULL	plasma concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a prospective study from 1991-1998 plasma concentrations of alpha-Tocopherole ( VitE ) and Selenium ( Se ) were analyzed in 125 sheep and 32 goats with generalised motor disturbances or elevated plasma-activities of Creatine-Kinase ( CK ) .
	manualset3
90665	4	399804	5	NULL	NULL	0	NULL	alpha-Tocopherole ( VitE )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In a prospective study from 1991-1998 plasma concentrations of alpha-Tocopherole ( VitE ) and Selenium ( Se ) were analyzed in 125 sheep and 32 goats with generalised motor disturbances or elevated plasma-activities of Creatine-Kinase ( CK ) .
	manualset3
90666	5	399804	5	NULL	NULL	0	NULL	Selenium ( Se )	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	In a prospective study from 1991-1998 plasma concentrations of alpha-Tocopherole ( VitE ) and Selenium ( Se ) were analyzed in 125 sheep and 32 goats with generalised motor disturbances or elevated plasma-activities of Creatine-Kinase ( CK ) .
	manualset3
90667	6	399804	5	NULL	NULL	0	NULL	125 sheep	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In a prospective study from 1991-1998 plasma concentrations of alpha-Tocopherole ( VitE ) and Selenium ( Se ) were analyzed in 125 sheep and 32 goats with generalised motor disturbances or elevated plasma-activities of Creatine-Kinase ( CK ) .
	manualset3
90668	7	399804	5	NULL	NULL	0	NULL	32 goats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In a prospective study from 1991-1998 plasma concentrations of alpha-Tocopherole ( VitE ) and Selenium ( Se ) were analyzed in 125 sheep and 32 goats with generalised motor disturbances or elevated plasma-activities of Creatine-Kinase ( CK ) .
	manualset3
90669	8	399804	5	NULL	NULL	0	NULL	generalised motor disturbances	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In a prospective study from 1991-1998 plasma concentrations of alpha-Tocopherole ( VitE ) and Selenium ( Se ) were analyzed in 125 sheep and 32 goats with generalised motor disturbances or elevated plasma-activities of Creatine-Kinase ( CK ) .
	manualset3
90670	9	399804	5	NULL	NULL	0	NULL	elevated plasma-activities of Creatine-Kinase ( CK )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In a prospective study from 1991-1998 plasma concentrations of alpha-Tocopherole ( VitE ) and Selenium ( Se ) were analyzed in 125 sheep and 32 goats with generalised motor disturbances or elevated plasma-activities of Creatine-Kinase ( CK ) .
	manualset3
90671	1	399805	5	NULL	NULL	0	NULL	randomized crossover study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a randomized crossover study , we compared the effects of a low-fat ( 30 % of daily energy ) diet and a high-fat ( 40 % of daily energy ) , high-monounsaturated-fat diet for 6 weeks each on fasting and postprandial glucose , insulin , and lipoprotein concentrations in 12 patients with well-controlled type 2 DM ( fasting blood glucose , 176 + / - 54 mg/dL ; hemoglobin A1c , 6.4 % + / - 0.7 % ) and no overt dyslipidemia ( serum total cholesterol , 235 + / - 43 mg/dL ; triglycerides , 180 + / - 63 mg/dL ) .
	manualset3
90672	2	399805	5	NULL	NULL	0	NULL	effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In a randomized crossover study , we compared the effects of a low-fat ( 30 % of daily energy ) diet and a high-fat ( 40 % of daily energy ) , high-monounsaturated-fat diet for 6 weeks each on fasting and postprandial glucose , insulin , and lipoprotein concentrations in 12 patients with well-controlled type 2 DM ( fasting blood glucose , 176 + / - 54 mg/dL ; hemoglobin A1c , 6.4 % + / - 0.7 % ) and no overt dyslipidemia ( serum total cholesterol , 235 + / - 43 mg/dL ; triglycerides , 180 + / - 63 mg/dL ) .
	manualset3
90673	3	399805	5	NULL	NULL	0	NULL	 low-fat ( 30 % of daily energy ) diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	In a randomized crossover study , we compared the effects of a low-fat ( 30 % of daily energy ) diet and a high-fat ( 40 % of daily energy ) , high-monounsaturated-fat diet for 6 weeks each on fasting and postprandial glucose , insulin , and lipoprotein concentrations in 12 patients with well-controlled type 2 DM ( fasting blood glucose , 176 + / - 54 mg/dL ; hemoglobin A1c , 6.4 % + / - 0.7 % ) and no overt dyslipidemia ( serum total cholesterol , 235 + / - 43 mg/dL ; triglycerides , 180 + / - 63 mg/dL ) .
	manualset3
90674	4	399805	5	NULL	NULL	0	NULL	high-fat ( 40 % of daily energy ) , high-monounsaturated-fat diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	In a randomized crossover study , we compared the effects of a low-fat ( 30 % of daily energy ) diet and a high-fat ( 40 % of daily energy ) , high-monounsaturated-fat diet for 6 weeks each on fasting and postprandial glucose , insulin , and lipoprotein concentrations in 12 patients with well-controlled type 2 DM ( fasting blood glucose , 176 + / - 54 mg/dL ; hemoglobin A1c , 6.4 % + / - 0.7 % ) and no overt dyslipidemia ( serum total cholesterol , 235 + / - 43 mg/dL ; triglycerides , 180 + / - 63 mg/dL ) .
	manualset3
90675	5	399805	5	NULL	NULL	0	NULL	6 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In a randomized crossover study , we compared the effects of a low-fat ( 30 % of daily energy ) diet and a high-fat ( 40 % of daily energy ) , high-monounsaturated-fat diet for 6 weeks each on fasting and postprandial glucose , insulin , and lipoprotein concentrations in 12 patients with well-controlled type 2 DM ( fasting blood glucose , 176 + / - 54 mg/dL ; hemoglobin A1c , 6.4 % + / - 0.7 % ) and no overt dyslipidemia ( serum total cholesterol , 235 + / - 43 mg/dL ; triglycerides , 180 + / - 63 mg/dL ) .
	manualset3
90676	6	399805	5	NULL	NULL	0	NULL	fasting	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In a randomized crossover study , we compared the effects of a low-fat ( 30 % of daily energy ) diet and a high-fat ( 40 % of daily energy ) , high-monounsaturated-fat diet for 6 weeks each on fasting and postprandial glucose , insulin , and lipoprotein concentrations in 12 patients with well-controlled type 2 DM ( fasting blood glucose , 176 + / - 54 mg/dL ; hemoglobin A1c , 6.4 % + / - 0.7 % ) and no overt dyslipidemia ( serum total cholesterol , 235 + / - 43 mg/dL ; triglycerides , 180 + / - 63 mg/dL ) .
	manualset3
90677	7	399805	5	NULL	NULL	0	NULL	postprandial glucose , insulin , and lipoprotein concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a randomized crossover study , we compared the effects of a low-fat ( 30 % of daily energy ) diet and a high-fat ( 40 % of daily energy ) , high-monounsaturated-fat diet for 6 weeks each on fasting and postprandial glucose , insulin , and lipoprotein concentrations in 12 patients with well-controlled type 2 DM ( fasting blood glucose , 176 + / - 54 mg/dL ; hemoglobin A1c , 6.4 % + / - 0.7 % ) and no overt dyslipidemia ( serum total cholesterol , 235 + / - 43 mg/dL ; triglycerides , 180 + / - 63 mg/dL ) .
	manualset3
90678	8	399805	5	NULL	NULL	NULL	NULL	12 patients with well-controlled type 2 DM 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a randomized crossover study , we compared the effects of a low-fat ( 30 % of daily energy ) diet and a high-fat ( 40 % of daily energy ) , high-monounsaturated-fat diet for 6 weeks each on fasting and postprandial glucose , insulin , and lipoprotein concentrations in 12 patients with well-controlled type 2 DM ( fasting blood glucose , 176 + / - 54 mg/dL ; hemoglobin A1c , 6.4 % + / - 0.7 % ) and no overt dyslipidemia ( serum total cholesterol , 235 + / - 43 mg/dL ; triglycerides , 180 + / - 63 mg/dL ) .
	manualset3
90680	9	399805	5	NULL	NULL	NULL	NULL	fasting blood glucose , 176 + / - 54 mg/dL	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a randomized crossover study , we compared the effects of a low-fat ( 30 % of daily energy ) diet and a high-fat ( 40 % of daily energy ) , high-monounsaturated-fat diet for 6 weeks each on fasting and postprandial glucose , insulin , and lipoprotein concentrations in 12 patients with well-controlled type 2 DM ( fasting blood glucose , 176 + / - 54 mg/dL ; hemoglobin A1c , 6.4 % + / - 0.7 % ) and no overt dyslipidemia ( serum total cholesterol , 235 + / - 43 mg/dL ; triglycerides , 180 + / - 63 mg/dL ) .
	manualset3
90681	10	399805	5	NULL	NULL	NULL	NULL	hemoglobin A1c , 6.4 % + / - 0.7 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a randomized crossover study , we compared the effects of a low-fat ( 30 % of daily energy ) diet and a high-fat ( 40 % of daily energy ) , high-monounsaturated-fat diet for 6 weeks each on fasting and postprandial glucose , insulin , and lipoprotein concentrations in 12 patients with well-controlled type 2 DM ( fasting blood glucose , 176 + / - 54 mg/dL ; hemoglobin A1c , 6.4 % + / - 0.7 % ) and no overt dyslipidemia ( serum total cholesterol , 235 + / - 43 mg/dL ; triglycerides , 180 + / - 63 mg/dL ) .
	manualset3
90682	11	399805	5	NULL	NULL	0	NULL	12 patients with no overt dyslipidemia	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In a randomized crossover study , we compared the effects of a low-fat ( 30 % of daily energy ) diet and a high-fat ( 40 % of daily energy ) , high-monounsaturated-fat diet for 6 weeks each on fasting and postprandial glucose , insulin , and lipoprotein concentrations in 12 patients with well-controlled type 2 DM ( fasting blood glucose , 176 + / - 54 mg/dL ; hemoglobin A1c , 6.4 % + / - 0.7 % ) and no overt dyslipidemia ( serum total cholesterol , 235 + / - 43 mg/dL ; triglycerides , 180 + / - 63 mg/dL ) .
	manualset3
90683	12	399805	5	NULL	NULL	0	NULL	 serum total cholesterol , 235 + / - 43 mg/dL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In a randomized crossover study , we compared the effects of a low-fat ( 30 % of daily energy ) diet and a high-fat ( 40 % of daily energy ) , high-monounsaturated-fat diet for 6 weeks each on fasting and postprandial glucose , insulin , and lipoprotein concentrations in 12 patients with well-controlled type 2 DM ( fasting blood glucose , 176 + / - 54 mg/dL ; hemoglobin A1c , 6.4 % + / - 0.7 % ) and no overt dyslipidemia ( serum total cholesterol , 235 + / - 43 mg/dL ; triglycerides , 180 + / - 63 mg/dL ) .
	manualset3
90684	13	399805	5	NULL	NULL	0	NULL	 triglycerides , 180 + / - 63 mg/dL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In a randomized crossover study , we compared the effects of a low-fat ( 30 % of daily energy ) diet and a high-fat ( 40 % of daily energy ) , high-monounsaturated-fat diet for 6 weeks each on fasting and postprandial glucose , insulin , and lipoprotein concentrations in 12 patients with well-controlled type 2 DM ( fasting blood glucose , 176 + / - 54 mg/dL ; hemoglobin A1c , 6.4 % + / - 0.7 % ) and no overt dyslipidemia ( serum total cholesterol , 235 + / - 43 mg/dL ; triglycerides , 180 + / - 63 mg/dL ) .
	manualset3
90685	1	399806	5	NULL	NULL	0	NULL	randomized trial	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a randomized trial of neurosurgical patients , groups wearing graduated compression stockings alone ( group 1 ) or graduated compression stockings plus intermittent pneumatic compression ( IPC ) ( group 2 ) were compared with an untreated control group in the prevention of deep vein thrombosis ( DVT ) .
	manualset3
90686	2	399806	5	NULL	NULL	0	NULL	neurosurgical patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In a randomized trial of neurosurgical patients , groups wearing graduated compression stockings alone ( group 1 ) or graduated compression stockings plus intermittent pneumatic compression ( IPC ) ( group 2 ) were compared with an untreated control group in the prevention of deep vein thrombosis ( DVT ) .
	manualset3
90687	3	399806	5	NULL	NULL	0	NULL	groups wearing graduated compression stockings alone ( group 1 )	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In a randomized trial of neurosurgical patients , groups wearing graduated compression stockings alone ( group 1 ) or graduated compression stockings plus intermittent pneumatic compression ( IPC ) ( group 2 ) were compared with an untreated control group in the prevention of deep vein thrombosis ( DVT ) .
	manualset3
90688	4	399806	5	NULL	NULL	0	NULL	groups wearing graduated compression stockings plus intermittent pneumatic compression ( IPC ) ( group 2 )	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In a randomized trial of neurosurgical patients , groups wearing graduated compression stockings alone ( group 1 ) or graduated compression stockings plus intermittent pneumatic compression ( IPC ) ( group 2 ) were compared with an untreated control group in the prevention of deep vein thrombosis ( DVT ) .
	manualset3
90689	5	399806	5	NULL	NULL	0	NULL	untreated control group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In a randomized trial of neurosurgical patients , groups wearing graduated compression stockings alone ( group 1 ) or graduated compression stockings plus intermittent pneumatic compression ( IPC ) ( group 2 ) were compared with an untreated control group in the prevention of deep vein thrombosis ( DVT ) .
	manualset3
90690	6	399806	5	NULL	NULL	0	NULL	prevention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In a randomized trial of neurosurgical patients , groups wearing graduated compression stockings alone ( group 1 ) or graduated compression stockings plus intermittent pneumatic compression ( IPC ) ( group 2 ) were compared with an untreated control group in the prevention of deep vein thrombosis ( DVT ) .
	manualset3
90691	7	399806	5	NULL	NULL	0	NULL	deep vein thrombosis ( DVT )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In a randomized trial of neurosurgical patients , groups wearing graduated compression stockings alone ( group 1 ) or graduated compression stockings plus intermittent pneumatic compression ( IPC ) ( group 2 ) were compared with an untreated control group in the prevention of deep vein thrombosis ( DVT ) .
	manualset3
90692	1	399807	5	NULL	NULL	NULL	NULL	response to comments	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a response to comments by P. T. Costa , Jr. , and R. R. McCrae on the current authors ' original article , the authors show that Costa and McCrae 's writings on personality suggest a belief in immutability of personality traits .
	manualset3
90693	2	399807	5	NULL	NULL	0	NULL	P. T. Costa , Jr.	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In a response to comments by P. T. Costa , Jr. , and R. R. McCrae on the current authors ' original article , the authors show that Costa and McCrae 's writings on personality suggest a belief in immutability of personality traits .
	manualset3
90694	3	399807	5	NULL	NULL	0	NULL	R. R. McCrae	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In a response to comments by P. T. Costa , Jr. , and R. R. McCrae on the current authors ' original article , the authors show that Costa and McCrae 's writings on personality suggest a belief in immutability of personality traits .
	manualset3
90695	4	399807	5	NULL	NULL	0	NULL	current authors ' original article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In a response to comments by P. T. Costa , Jr. , and R. R. McCrae on the current authors ' original article , the authors show that Costa and McCrae 's writings on personality suggest a belief in immutability of personality traits .
	manualset3
90696	5	399807	5	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In a response to comments by P. T. Costa , Jr. , and R. R. McCrae on the current authors ' original article , the authors show that Costa and McCrae 's writings on personality suggest a belief in immutability of personality traits .
	manualset3
90697	6	399807	5	NULL	NULL	NULL	NULL	Costa and McCrae 's writings on personality	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a response to comments by P. T. Costa , Jr. , and R. R. McCrae on the current authors ' original article , the authors show that Costa and McCrae 's writings on personality suggest a belief in immutability of personality traits .
	manualset3
90698	7	399807	5	NULL	NULL	0	NULL	immutability of personality traits	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In a response to comments by P. T. Costa , Jr. , and R. R. McCrae on the current authors ' original article , the authors show that Costa and McCrae 's writings on personality suggest a belief in immutability of personality traits .
	manualset3
90699	1	399808	5	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In a review the prognostic value of such tests is discussed and shown , that in spite of partially high prediction rates , the prognostic value of either S. mutans or Lactobacillus tests can be confirmed only in combination with additional relevant clinical parameters ( e.g. anamnesis , DMF-increment , secretation rate and bufferin capacity of saliva ... ) .
	manualset3
90700	2	399808	5	NULL	NULL	0	NULL	prognostic value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a review the prognostic value of such tests is discussed and shown , that in spite of partially high prediction rates , the prognostic value of either S. mutans or Lactobacillus tests can be confirmed only in combination with additional relevant clinical parameters ( e.g. anamnesis , DMF-increment , secretation rate and bufferin capacity of saliva ... ) .
	manualset3
90701	3	399808	5	NULL	NULL	0	NULL	tests	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a review the prognostic value of such tests is discussed and shown , that in spite of partially high prediction rates , the prognostic value of either S. mutans or Lactobacillus tests can be confirmed only in combination with additional relevant clinical parameters ( e.g. anamnesis , DMF-increment , secretation rate and bufferin capacity of saliva ... ) .
	manualset3
90702	4	399808	5	NULL	NULL	0	NULL	partially high prediction rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a review the prognostic value of such tests is discussed and shown , that in spite of partially high prediction rates , the prognostic value of either S. mutans or Lactobacillus tests can be confirmed only in combination with additional relevant clinical parameters ( e.g. anamnesis , DMF-increment , secretation rate and bufferin capacity of saliva ... ) .
	manualset3
90703	5	399808	5	NULL	NULL	0	NULL	prognostic value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a review the prognostic value of such tests is discussed and shown , that in spite of partially high prediction rates , the prognostic value of either S. mutans or Lactobacillus tests can be confirmed only in combination with additional relevant clinical parameters ( e.g. anamnesis , DMF-increment , secretation rate and bufferin capacity of saliva ... ) .
	manualset3
90704	6	399808	5	NULL	NULL	0	NULL	S. mutans or Lactobacillus tests	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a review the prognostic value of such tests is discussed and shown , that in spite of partially high prediction rates , the prognostic value of either S. mutans or Lactobacillus tests can be confirmed only in combination with additional relevant clinical parameters ( e.g. anamnesis , DMF-increment , secretation rate and bufferin capacity of saliva ... ) .
	manualset3
90705	7	399808	5	NULL	NULL	NULL	NULL	additional relevant clinical parameters	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a review the prognostic value of such tests is discussed and shown , that in spite of partially high prediction rates , the prognostic value of either S. mutans or Lactobacillus tests can be confirmed only in combination with additional relevant clinical parameters ( e.g. anamnesis , DMF-increment , secretation rate and bufferin capacity of saliva ... ) .
	manualset3
90706	8	399808	5	NULL	NULL	0	NULL	anamnesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In a review the prognostic value of such tests is discussed and shown , that in spite of partially high prediction rates , the prognostic value of either S. mutans or Lactobacillus tests can be confirmed only in combination with additional relevant clinical parameters ( e.g. anamnesis , DMF-increment , secretation rate and bufferin capacity of saliva ... ) .
	manualset3
90707	9	399808	5	NULL	NULL	0	NULL	DMF-increment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In a review the prognostic value of such tests is discussed and shown , that in spite of partially high prediction rates , the prognostic value of either S. mutans or Lactobacillus tests can be confirmed only in combination with additional relevant clinical parameters ( e.g. anamnesis , DMF-increment , secretation rate and bufferin capacity of saliva ... ) .
	manualset3
90708	10	399808	5	NULL	NULL	0	NULL	secretation rate and bufferin capacity of saliva 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In a review the prognostic value of such tests is discussed and shown , that in spite of partially high prediction rates , the prognostic value of either S. mutans or Lactobacillus tests can be confirmed only in combination with additional relevant clinical parameters ( e.g. anamnesis , DMF-increment , secretation rate and bufferin capacity of saliva ... ) .
	manualset3
90709	1	399809	5	NULL	NULL	0	NULL	second experiment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a second experiment , development of embryos was similar after co-culture on OM or STO cells for both 3 and 6 days .
	manualset3
90710	2	399809	5	NULL	NULL	0	NULL	development of embryos	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In a second experiment , development of embryos was similar after co-culture on OM or STO cells for both 3 and 6 days .
	manualset3
90711	3	399809	5	NULL	NULL	0	NULL	co-culture	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In a second experiment , development of embryos was similar after co-culture on OM or STO cells for both 3 and 6 days .
	manualset3
90712	4	399809	5	NULL	NULL	0	NULL	OM or STO cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In a second experiment , development of embryos was similar after co-culture on OM or STO cells for both 3 and 6 days .
	manualset3
90713	5	399809	5	NULL	NULL	0	NULL	3 and 6 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In a second experiment , development of embryos was similar after co-culture on OM or STO cells for both 3 and 6 days .
	manualset3
90714	1	399810	5	NULL	NULL	0	NULL	second experiment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a second experiment , parasitism of Xa and Xr by Aph and Lep was increased when nematodes were incubated in 2 % soil extract for 4 days before exposure to zoospores .
	manualset3
90715	2	399810	5	NULL	NULL	0	NULL	parasitism of Xa and Xr by Aph and Lep	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In a second experiment , parasitism of Xa and Xr by Aph and Lep was increased when nematodes were incubated in 2 % soil extract for 4 days before exposure to zoospores .
	manualset3
90716	3	399810	5	NULL	NULL	0	NULL	nematodes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In a second experiment , parasitism of Xa and Xr by Aph and Lep was increased when nematodes were incubated in 2 % soil extract for 4 days before exposure to zoospores .
	manualset3
90717	4	399810	5	NULL	NULL	0	NULL	2 % soil extract	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In a second experiment , parasitism of Xa and Xr by Aph and Lep was increased when nematodes were incubated in 2 % soil extract for 4 days before exposure to zoospores .
	manualset3
90718	5	399810	5	NULL	NULL	0	NULL	4 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In a second experiment , parasitism of Xa and Xr by Aph and Lep was increased when nematodes were incubated in 2 % soil extract for 4 days before exposure to zoospores .
	manualset3
90719	6	399810	5	NULL	NULL	0	NULL	exposure to zoospores	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a second experiment , parasitism of Xa and Xr by Aph and Lep was increased when nematodes were incubated in 2 % soil extract for 4 days before exposure to zoospores .
	manualset3
90720	1	399811	5	NULL	NULL	0	NULL	second experiment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a second experiment , stained linear 48.5 kbp DNA molecules are observed as random coils immobilized in agarose .
	manualset3
90721	2	399811	5	NULL	NULL	0	NULL	stained linear 48.5 kbp DNA molecules	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In a second experiment , stained linear 48.5 kbp DNA molecules are observed as random coils immobilized in agarose .
	manualset3
90722	3	399811	5	NULL	NULL	0	NULL	random coils	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In a second experiment , stained linear 48.5 kbp DNA molecules are observed as random coils immobilized in agarose .
	manualset3
90723	4	399811	5	NULL	NULL	0	NULL	agarose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In a second experiment , stained linear 48.5 kbp DNA molecules are observed as random coils immobilized in agarose .
	manualset3
90724	1	399812	5	NULL	NULL	0	NULL	selective attention task	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a selective attention task , 21 Subjects detected rare randomized targets ( P = 0.02 ) in a set of randomized standard tones .
	manualset3
90725	2	399812	5	NULL	NULL	0	NULL	21 Subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In a selective attention task , 21 Subjects detected rare randomized targets ( P = 0.02 ) in a set of randomized standard tones .
	manualset3
90726	3	399812	5	NULL	NULL	0	NULL	rare randomized targets	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a selective attention task , 21 Subjects detected rare randomized targets ( P = 0.02 ) in a set of randomized standard tones .
	manualset3
90727	4	399812	5	NULL	NULL	0	NULL	P = 0.02	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In a selective attention task , 21 Subjects detected rare randomized targets ( P = 0.02 ) in a set of randomized standard tones .
	manualset3
90728	5	399812	5	NULL	NULL	0	NULL	set of randomized standard tones	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a selective attention task , 21 Subjects detected rare randomized targets ( P = 0.02 ) in a set of randomized standard tones .
	manualset3
90729	1	399813	5	NULL	NULL	0	NULL	Ultracytochemical localisation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Ultracytochemical localisation of the alkaline phosphatase in the cerebral cortex of newborn rats ( author 's transl ) ) .
	manualset3
90730	2	399813	5	NULL	NULL	0	NULL	alkaline phosphatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Ultracytochemical localisation of the alkaline phosphatase in the cerebral cortex of newborn rats ( author 's transl ) ) .
	manualset3
90731	3	399813	5	NULL	NULL	0	NULL	cerebral cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Ultracytochemical localisation of the alkaline phosphatase in the cerebral cortex of newborn rats ( author 's transl ) ) .
	manualset3
90732	4	399813	5	NULL	NULL	0	NULL	newborn rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Ultracytochemical localisation of the alkaline phosphatase in the cerebral cortex of newborn rats ( author 's transl ) ) .
	manualset3
90733	1	399814	5	NULL	NULL	0	NULL	separate series of experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a separate series of experiments a GAG fraction was isolated from transport labeled SPM and was found to consist of heparan sulfate containing 28 % of transported radioactivity .
	manualset3
90734	2	399814	5	NULL	NULL	0	NULL	GAG fraction	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In a separate series of experiments a GAG fraction was isolated from transport labeled SPM and was found to consist of heparan sulfate containing 28 % of transported radioactivity .
	manualset3
90735	3	399814	5	NULL	NULL	0	NULL	transport labeled SPM	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In a separate series of experiments a GAG fraction was isolated from transport labeled SPM and was found to consist of heparan sulfate containing 28 % of transported radioactivity .
	manualset3
90736	4	399814	5	NULL	NULL	0	NULL	heparan sulfate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In a separate series of experiments a GAG fraction was isolated from transport labeled SPM and was found to consist of heparan sulfate containing 28 % of transported radioactivity .
	manualset3
90737	5	399814	5	NULL	NULL	0	NULL	 28 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In a separate series of experiments a GAG fraction was isolated from transport labeled SPM and was found to consist of heparan sulfate containing 28 % of transported radioactivity .
	manualset3
90738	6	399814	5	NULL	NULL	0	NULL	transported radioactivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In a separate series of experiments a GAG fraction was isolated from transport labeled SPM and was found to consist of heparan sulfate containing 28 % of transported radioactivity .
	manualset3
90747	1	399815	5	NULL	NULL	0	NULL	series of 6 experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a series of 6 experiments with CD8F1 mice with spontaneous mammary adenocarcinomas Sugiura noted by macrovisual observation with some histology an overall average of 21 % of mice with lung metastases when treated with 1 , 000 -- 2 , 000 mg/kg/day of amygdalin compared with 90 % of the control mice .
	manualset3
90748	2	399815	5	NULL	NULL	0	NULL	CD8F1 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In a series of 6 experiments with CD8F1 mice with spontaneous mammary adenocarcinomas Sugiura noted by macrovisual observation with some histology an overall average of 21 % of mice with lung metastases when treated with 1 , 000 -- 2 , 000 mg/kg/day of amygdalin compared with 90 % of the control mice .
	manualset3
90753	3	399815	5	NULL	NULL	0	NULL	spontaneous mammary adenocarcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In a series of 6 experiments with CD8F1 mice with spontaneous mammary adenocarcinomas Sugiura noted by macrovisual observation with some histology an overall average of 21 % of mice with lung metastases when treated with 1 , 000 -- 2 , 000 mg/kg/day of amygdalin compared with 90 % of the control mice .
	manualset3
90754	4	399815	5	NULL	NULL	0	NULL	Sugiura	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In a series of 6 experiments with CD8F1 mice with spontaneous mammary adenocarcinomas Sugiura noted by macrovisual observation with some histology an overall average of 21 % of mice with lung metastases when treated with 1 , 000 -- 2 , 000 mg/kg/day of amygdalin compared with 90 % of the control mice .
	manualset3
90756	5	399815	5	NULL	NULL	0	NULL	macrovisual observation with some histology	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a series of 6 experiments with CD8F1 mice with spontaneous mammary adenocarcinomas Sugiura noted by macrovisual observation with some histology an overall average of 21 % of mice with lung metastases when treated with 1 , 000 -- 2 , 000 mg/kg/day of amygdalin compared with 90 % of the control mice .
	manualset3
90757	6	399815	5	NULL	NULL	0	NULL	21 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In a series of 6 experiments with CD8F1 mice with spontaneous mammary adenocarcinomas Sugiura noted by macrovisual observation with some histology an overall average of 21 % of mice with lung metastases when treated with 1 , 000 -- 2 , 000 mg/kg/day of amygdalin compared with 90 % of the control mice .
	manualset3
90758	7	399815	5	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In a series of 6 experiments with CD8F1 mice with spontaneous mammary adenocarcinomas Sugiura noted by macrovisual observation with some histology an overall average of 21 % of mice with lung metastases when treated with 1 , 000 -- 2 , 000 mg/kg/day of amygdalin compared with 90 % of the control mice .
	manualset3
90759	8	399815	5	NULL	NULL	0	NULL	lung metastases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In a series of 6 experiments with CD8F1 mice with spontaneous mammary adenocarcinomas Sugiura noted by macrovisual observation with some histology an overall average of 21 % of mice with lung metastases when treated with 1 , 000 -- 2 , 000 mg/kg/day of amygdalin compared with 90 % of the control mice .
	manualset3
90760	9	399815	5	NULL	NULL	0	NULL	1 , 000 -- 2 , 000 mg/kg/day	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In a series of 6 experiments with CD8F1 mice with spontaneous mammary adenocarcinomas Sugiura noted by macrovisual observation with some histology an overall average of 21 % of mice with lung metastases when treated with 1 , 000 -- 2 , 000 mg/kg/day of amygdalin compared with 90 % of the control mice .
	manualset3
90762	10	399815	5	NULL	NULL	0	NULL	90 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In a series of 6 experiments with CD8F1 mice with spontaneous mammary adenocarcinomas Sugiura noted by macrovisual observation with some histology an overall average of 21 % of mice with lung metastases when treated with 1 , 000 -- 2 , 000 mg/kg/day of amygdalin compared with 90 % of the control mice .
	manualset3
90764	11	399815	5	NULL	NULL	0	NULL	control mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In a series of 6 experiments with CD8F1 mice with spontaneous mammary adenocarcinomas Sugiura noted by macrovisual observation with some histology an overall average of 21 % of mice with lung metastases when treated with 1 , 000 -- 2 , 000 mg/kg/day of amygdalin compared with 90 % of the control mice .
	manualset3
90765	1	399816	5	NULL	NULL	0	NULL	series of experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a series of experiments , we applied the ` taste reactivity ' measure of affective reactions ( gapes , etc. ) to assess the capacity of dopamine-depleted rats for : 1 ) normal affect ( hedonic and aversive reactions ) , 2 ) modulation of hedonic affect by associative learning ( taste aversion conditioning ) , and 3 ) hedonic enhancement of affect by non-dopaminergic pharmacological manipulation of palatability ( benzodiazepine administration ) .
	manualset3
91065	2	399816	5	NULL	NULL	NULL	NULL	` taste reactivity ' 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a series of experiments , we applied the ` taste reactivity ' measure of affective reactions ( gapes , etc. ) to assess the capacity of dopamine-depleted rats for : 1 ) normal affect ( hedonic and aversive reactions ) , 2 ) modulation of hedonic affect by associative learning ( taste aversion conditioning ) , and 3 ) hedonic enhancement of affect by non-dopaminergic pharmacological manipulation of palatability ( benzodiazepine administration ) .
	manualset3
91066	3	399816	5	NULL	NULL	0	NULL	measure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a series of experiments , we applied the ` taste reactivity ' measure of affective reactions ( gapes , etc. ) to assess the capacity of dopamine-depleted rats for : 1 ) normal affect ( hedonic and aversive reactions ) , 2 ) modulation of hedonic affect by associative learning ( taste aversion conditioning ) , and 3 ) hedonic enhancement of affect by non-dopaminergic pharmacological manipulation of palatability ( benzodiazepine administration ) .
	manualset3
91067	4	399816	5	NULL	NULL	0	NULL	affective reactions ( gapes , etc. )	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In a series of experiments , we applied the ` taste reactivity ' measure of affective reactions ( gapes , etc. ) to assess the capacity of dopamine-depleted rats for : 1 ) normal affect ( hedonic and aversive reactions ) , 2 ) modulation of hedonic affect by associative learning ( taste aversion conditioning ) , and 3 ) hedonic enhancement of affect by non-dopaminergic pharmacological manipulation of palatability ( benzodiazepine administration ) .
	manualset3
91068	5	399816	5	NULL	NULL	0	NULL	capacity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a series of experiments , we applied the ` taste reactivity ' measure of affective reactions ( gapes , etc. ) to assess the capacity of dopamine-depleted rats for : 1 ) normal affect ( hedonic and aversive reactions ) , 2 ) modulation of hedonic affect by associative learning ( taste aversion conditioning ) , and 3 ) hedonic enhancement of affect by non-dopaminergic pharmacological manipulation of palatability ( benzodiazepine administration ) .
	manualset3
91069	6	399816	5	NULL	NULL	0	NULL	dopamine-depleted rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In a series of experiments , we applied the ` taste reactivity ' measure of affective reactions ( gapes , etc. ) to assess the capacity of dopamine-depleted rats for : 1 ) normal affect ( hedonic and aversive reactions ) , 2 ) modulation of hedonic affect by associative learning ( taste aversion conditioning ) , and 3 ) hedonic enhancement of affect by non-dopaminergic pharmacological manipulation of palatability ( benzodiazepine administration ) .
	manualset3
91070	7	399816	5	NULL	NULL	0	NULL	normal affect ( hedonic and aversive reactions )	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In a series of experiments , we applied the ` taste reactivity ' measure of affective reactions ( gapes , etc. ) to assess the capacity of dopamine-depleted rats for : 1 ) normal affect ( hedonic and aversive reactions ) , 2 ) modulation of hedonic affect by associative learning ( taste aversion conditioning ) , and 3 ) hedonic enhancement of affect by non-dopaminergic pharmacological manipulation of palatability ( benzodiazepine administration ) .
	manualset3
91071	8	399816	5	NULL	NULL	0	NULL	modulation of hedonic affect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In a series of experiments , we applied the ` taste reactivity ' measure of affective reactions ( gapes , etc. ) to assess the capacity of dopamine-depleted rats for : 1 ) normal affect ( hedonic and aversive reactions ) , 2 ) modulation of hedonic affect by associative learning ( taste aversion conditioning ) , and 3 ) hedonic enhancement of affect by non-dopaminergic pharmacological manipulation of palatability ( benzodiazepine administration ) .
	manualset3
91072	9	399816	5	NULL	NULL	0	NULL	associative learning ( taste aversion conditioning )	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In a series of experiments , we applied the ` taste reactivity ' measure of affective reactions ( gapes , etc. ) to assess the capacity of dopamine-depleted rats for : 1 ) normal affect ( hedonic and aversive reactions ) , 2 ) modulation of hedonic affect by associative learning ( taste aversion conditioning ) , and 3 ) hedonic enhancement of affect by non-dopaminergic pharmacological manipulation of palatability ( benzodiazepine administration ) .
	manualset3
91073	10	399816	5	NULL	NULL	0	NULL	hedonic enhancement of affect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In a series of experiments , we applied the ` taste reactivity ' measure of affective reactions ( gapes , etc. ) to assess the capacity of dopamine-depleted rats for : 1 ) normal affect ( hedonic and aversive reactions ) , 2 ) modulation of hedonic affect by associative learning ( taste aversion conditioning ) , and 3 ) hedonic enhancement of affect by non-dopaminergic pharmacological manipulation of palatability ( benzodiazepine administration ) .
	manualset3
91074	11	399816	5	NULL	NULL	NULL	NULL	non-dopaminergic pharmacological manipulation of palatability	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a series of experiments , we applied the ` taste reactivity ' measure of affective reactions ( gapes , etc. ) to assess the capacity of dopamine-depleted rats for : 1 ) normal affect ( hedonic and aversive reactions ) , 2 ) modulation of hedonic affect by associative learning ( taste aversion conditioning ) , and 3 ) hedonic enhancement of affect by non-dopaminergic pharmacological manipulation of palatability ( benzodiazepine administration ) .
	manualset3
91075	12	399816	5	NULL	NULL	NULL	NULL	benzodiazepine administration	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a series of experiments , we applied the ` taste reactivity ' measure of affective reactions ( gapes , etc. ) to assess the capacity of dopamine-depleted rats for : 1 ) normal affect ( hedonic and aversive reactions ) , 2 ) modulation of hedonic affect by associative learning ( taste aversion conditioning ) , and 3 ) hedonic enhancement of affect by non-dopaminergic pharmacological manipulation of palatability ( benzodiazepine administration ) .
	manualset3
90973	1	399817	5	NULL	NULL	0	NULL	small number of patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In a small number of patients ( i.e. 17.8 % of macroprolactinomas and 10 % of microprolactinomas ) , however , CAB treatment did not normalize serum PRL levels despite reducing tumor mass , even at very high doses .
	manualset3
90974	2	399817	5	NULL	NULL	NULL	NULL	17.8 % of macroprolactinomas	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a small number of patients ( i.e. 17.8 % of macroprolactinomas and 10 % of microprolactinomas ) , however , CAB treatment did not normalize serum PRL levels despite reducing tumor mass , even at very high doses .
	manualset3
90975	3	399817	5	NULL	NULL	NULL	NULL	10 % of microprolactinomas	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a small number of patients ( i.e. 17.8 % of macroprolactinomas and 10 % of microprolactinomas ) , however , CAB treatment did not normalize serum PRL levels despite reducing tumor mass , even at very high doses .
	manualset3
90976	4	399817	5	NULL	NULL	0	NULL	CAB treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In a small number of patients ( i.e. 17.8 % of macroprolactinomas and 10 % of microprolactinomas ) , however , CAB treatment did not normalize serum PRL levels despite reducing tumor mass , even at very high doses .
	manualset3
90977	5	399817	5	NULL	NULL	0	NULL	serum PRL levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a small number of patients ( i.e. 17.8 % of macroprolactinomas and 10 % of microprolactinomas ) , however , CAB treatment did not normalize serum PRL levels despite reducing tumor mass , even at very high doses .
	manualset3
90978	6	399817	5	NULL	NULL	NULL	NULL	tumor mass	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a small number of patients ( i.e. 17.8 % of macroprolactinomas and 10 % of microprolactinomas ) , however , CAB treatment did not normalize serum PRL levels despite reducing tumor mass , even at very high doses .
	manualset3
90979	7	399817	5	NULL	NULL	0	NULL	very high doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a small number of patients ( i.e. 17.8 % of macroprolactinomas and 10 % of microprolactinomas ) , however , CAB treatment did not normalize serum PRL levels despite reducing tumor mass , even at very high doses .
	manualset3
90980	1	399818	5	NULL	NULL	0	NULL	small subset of taste cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In a small subset of taste cells , L-AP4 elicited an increase in holding current , resulting in taste cell depolarization under current clamp .
	manualset3
90981	2	399818	5	NULL	NULL	0	NULL	L-AP4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In a small subset of taste cells , L-AP4 elicited an increase in holding current , resulting in taste cell depolarization under current clamp .
	manualset3
90982	3	399818	5	NULL	NULL	0	NULL	holding current	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In a small subset of taste cells , L-AP4 elicited an increase in holding current , resulting in taste cell depolarization under current clamp .
	manualset3
90983	4	399818	5	NULL	NULL	0	NULL	taste cell depolarization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In a small subset of taste cells , L-AP4 elicited an increase in holding current , resulting in taste cell depolarization under current clamp .
	manualset3
90984	5	399818	5	NULL	NULL	NULL	NULL	current clamp	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a small subset of taste cells , L-AP4 elicited an increase in holding current , resulting in taste cell depolarization under current clamp .
	manualset3
90985	1	399819	5	NULL	NULL	0	NULL	standard ratio of tissue-air ratios ( RTAR ) algorithm	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In a standard ratio of tissue-air ratios ( RTAR ) algorithm , doses to points in irregular field geometries are not adequately modeled .
	manualset3
90986	2	399819	5	NULL	NULL	0	NULL	doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a standard ratio of tissue-air ratios ( RTAR ) algorithm , doses to points in irregular field geometries are not adequately modeled .
	manualset3
90987	3	399819	5	NULL	NULL	0	NULL	points	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a standard ratio of tissue-air ratios ( RTAR ) algorithm , doses to points in irregular field geometries are not adequately modeled .
	manualset3
90988	4	399819	5	NULL	NULL	0	NULL	irregular field geometries	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a standard ratio of tissue-air ratios ( RTAR ) algorithm , doses to points in irregular field geometries are not adequately modeled .
	manualset3
90989	1	399820	5	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a study of 20 patients diagnosed with malignant ovarian germ cell tumors between 1961 and 1993 , clinical and pathologic findings were evaluated .
	manualset3
90990	2	399820	5	NULL	NULL	0	NULL	20 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In a study of 20 patients diagnosed with malignant ovarian germ cell tumors between 1961 and 1993 , clinical and pathologic findings were evaluated .
	manualset3
90991	3	399820	5	NULL	NULL	0	NULL	malignant ovarian germ cell tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In a study of 20 patients diagnosed with malignant ovarian germ cell tumors between 1961 and 1993 , clinical and pathologic findings were evaluated .
	manualset3
90992	4	399820	5	NULL	NULL	0	NULL	between 1961 and 1993	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In a study of 20 patients diagnosed with malignant ovarian germ cell tumors between 1961 and 1993 , clinical and pathologic findings were evaluated .
	manualset3
90993	5	399820	5	NULL	NULL	0	NULL	clinical and pathologic findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In a study of 20 patients diagnosed with malignant ovarian germ cell tumors between 1961 and 1993 , clinical and pathologic findings were evaluated .
	manualset3
90994	1	399821	5	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a study of 34 adult gerbils exposed to such a procedure , 11 , or 33 % , developed severe neurological sequelae and succumbed to the procedure in less than 30 hr , whereas 23 animals survived with only minor or transient neurological signs .
	manualset3
90995	2	399821	5	NULL	NULL	0	NULL	34 adult gerbils	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In a study of 34 adult gerbils exposed to such a procedure , 11 , or 33 % , developed severe neurological sequelae and succumbed to the procedure in less than 30 hr , whereas 23 animals survived with only minor or transient neurological signs .
	manualset3
90996	3	399821	5	NULL	NULL	0	NULL	procedure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a study of 34 adult gerbils exposed to such a procedure , 11 , or 33 % , developed severe neurological sequelae and succumbed to the procedure in less than 30 hr , whereas 23 animals survived with only minor or transient neurological signs .
	manualset3
90997	4	399821	5	NULL	NULL	0	NULL	11 , or 33 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In a study of 34 adult gerbils exposed to such a procedure , 11 , or 33 % , developed severe neurological sequelae and succumbed to the procedure in less than 30 hr , whereas 23 animals survived with only minor or transient neurological signs .
	manualset3
90998	5	399821	5	NULL	NULL	0	NULL	severe neurological sequelae	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In a study of 34 adult gerbils exposed to such a procedure , 11 , or 33 % , developed severe neurological sequelae and succumbed to the procedure in less than 30 hr , whereas 23 animals survived with only minor or transient neurological signs .
	manualset3
90999	6	399821	5	NULL	NULL	0	NULL	procedure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a study of 34 adult gerbils exposed to such a procedure , 11 , or 33 % , developed severe neurological sequelae and succumbed to the procedure in less than 30 hr , whereas 23 animals survived with only minor or transient neurological signs .
	manualset3
91000	7	399821	5	NULL	NULL	0	NULL	less than 30 hr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In a study of 34 adult gerbils exposed to such a procedure , 11 , or 33 % , developed severe neurological sequelae and succumbed to the procedure in less than 30 hr , whereas 23 animals survived with only minor or transient neurological signs .
	manualset3
91001	8	399821	5	NULL	NULL	0	NULL	23 animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In a study of 34 adult gerbils exposed to such a procedure , 11 , or 33 % , developed severe neurological sequelae and succumbed to the procedure in less than 30 hr , whereas 23 animals survived with only minor or transient neurological signs .
	manualset3
91002	9	399821	5	NULL	NULL	0	NULL	minor or transient neurological signs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In a study of 34 adult gerbils exposed to such a procedure , 11 , or 33 % , developed severe neurological sequelae and succumbed to the procedure in less than 30 hr , whereas 23 animals survived with only minor or transient neurological signs .
	manualset3
91003	1	399822	5	NULL	NULL	0	NULL	subgroup of 22 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In a subgroup of 22 patients thought to be clinically stable , ROA was calculated serially over a mean follow-up period of 2 months and its variability compared with that of other flow-based parameters obtainable from proximal acceleration .
	manualset3
91005	2	399822	5	NULL	NULL	NULL	NULL	ROA	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a subgroup of 22 patients thought to be clinically stable , ROA was calculated serially over a mean follow-up period of 2 months and its variability compared with that of other flow-based parameters obtainable from proximal acceleration .
	manualset3
91006	3	399822	5	NULL	NULL	NULL	NULL	mean follow-up period	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a subgroup of 22 patients thought to be clinically stable , ROA was calculated serially over a mean follow-up period of 2 months and its variability compared with that of other flow-based parameters obtainable from proximal acceleration .
	manualset3
91007	4	399822	5	NULL	NULL	NULL	NULL	2 months	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a subgroup of 22 patients thought to be clinically stable , ROA was calculated serially over a mean follow-up period of 2 months and its variability compared with that of other flow-based parameters obtainable from proximal acceleration .
	manualset3
91008	5	399822	5	NULL	NULL	NULL	NULL	variability	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a subgroup of 22 patients thought to be clinically stable , ROA was calculated serially over a mean follow-up period of 2 months and its variability compared with that of other flow-based parameters obtainable from proximal acceleration .
	manualset3
91009	6	399822	5	NULL	NULL	NULL	NULL	flow-based parameters	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a subgroup of 22 patients thought to be clinically stable , ROA was calculated serially over a mean follow-up period of 2 months and its variability compared with that of other flow-based parameters obtainable from proximal acceleration .
	manualset3
91010	7	399822	5	NULL	NULL	NULL	NULL	proximal acceleration	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a subgroup of 22 patients thought to be clinically stable , ROA was calculated serially over a mean follow-up period of 2 months and its variability compared with that of other flow-based parameters obtainable from proximal acceleration .
	manualset3
91011	1	399823	5	NULL	NULL	0	NULL	subgroup of 25 OSA patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In a subgroup of 25 OSA patients reevaluated after at least 1 year of home treatment with nasal continuous positive airway pressure the reported frequency of nocturnal micturitions had significantly decreased ( p & lt ; 0.001 ) .
	manualset3
91012	2	399823	5	NULL	NULL	0	NULL	1 year	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In a subgroup of 25 OSA patients reevaluated after at least 1 year of home treatment with nasal continuous positive airway pressure the reported frequency of nocturnal micturitions had significantly decreased ( p & lt ; 0.001 ) .
	manualset3
91013	3	399823	5	NULL	NULL	0	NULL	home treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In a subgroup of 25 OSA patients reevaluated after at least 1 year of home treatment with nasal continuous positive airway pressure the reported frequency of nocturnal micturitions had significantly decreased ( p & lt ; 0.001 ) .
	manualset3
91014	4	399823	5	NULL	NULL	0	NULL	nasal continuous positive airway pressure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In a subgroup of 25 OSA patients reevaluated after at least 1 year of home treatment with nasal continuous positive airway pressure the reported frequency of nocturnal micturitions had significantly decreased ( p & lt ; 0.001 ) .
	manualset3
91015	5	399823	5	NULL	NULL	0	NULL	reported frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a subgroup of 25 OSA patients reevaluated after at least 1 year of home treatment with nasal continuous positive airway pressure the reported frequency of nocturnal micturitions had significantly decreased ( p & lt ; 0.001 ) .
	manualset3
91016	6	399823	5	NULL	NULL	0	NULL	nocturnal micturitions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In a subgroup of 25 OSA patients reevaluated after at least 1 year of home treatment with nasal continuous positive airway pressure the reported frequency of nocturnal micturitions had significantly decreased ( p & lt ; 0.001 ) .
	manualset3
91017	7	399823	5	NULL	NULL	0	NULL	p & lt ; 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In a subgroup of 25 OSA patients reevaluated after at least 1 year of home treatment with nasal continuous positive airway pressure the reported frequency of nocturnal micturitions had significantly decreased ( p & lt ; 0.001 ) .
	manualset3
91018	1	399824	5	NULL	NULL	0	NULL	Ultrasonics	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Ultrasonics and phonophoresis in the treatment of chronic pharyngitis ) .
	manualset3
91019	2	399824	5	NULL	NULL	0	NULL	phonophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Ultrasonics and phonophoresis in the treatment of chronic pharyngitis ) .
	manualset3
91020	3	399824	5	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Ultrasonics and phonophoresis in the treatment of chronic pharyngitis ) .
	manualset3
91021	4	399824	5	NULL	NULL	0	NULL	chronic pharyngitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Ultrasonics and phonophoresis in the treatment of chronic pharyngitis ) .
	manualset3
91022	1	399825	5	NULL	NULL	0	NULL	subgroup of 41 subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In a subgroup of 41 subjects whose primary tumors were allelotyped , the fractional allelic loss ( FAL ) at 39 autosomal arms also significantly correlated with disease-free survival ( P = 0.013 ) , with an increase in FAL associated with a poorer outcome ; this association remained significant when controlled for tumor thickness ( P = 0.035 ) .
	manualset3
91023	2	399825	5	NULL	NULL	0	NULL	primary tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In a subgroup of 41 subjects whose primary tumors were allelotyped , the fractional allelic loss ( FAL ) at 39 autosomal arms also significantly correlated with disease-free survival ( P = 0.013 ) , with an increase in FAL associated with a poorer outcome ; this association remained significant when controlled for tumor thickness ( P = 0.035 ) .
	manualset3
91025	3	399825	5	NULL	NULL	0	NULL	fractional allelic loss ( FAL )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a subgroup of 41 subjects whose primary tumors were allelotyped , the fractional allelic loss ( FAL ) at 39 autosomal arms also significantly correlated with disease-free survival ( P = 0.013 ) , with an increase in FAL associated with a poorer outcome ; this association remained significant when controlled for tumor thickness ( P = 0.035 ) .
	manualset3
91026	4	399825	5	NULL	NULL	0	NULL	39 autosomal arms	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	In a subgroup of 41 subjects whose primary tumors were allelotyped , the fractional allelic loss ( FAL ) at 39 autosomal arms also significantly correlated with disease-free survival ( P = 0.013 ) , with an increase in FAL associated with a poorer outcome ; this association remained significant when controlled for tumor thickness ( P = 0.035 ) .
	manualset3
91027	5	399825	5	NULL	NULL	0	NULL	disease-free survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In a subgroup of 41 subjects whose primary tumors were allelotyped , the fractional allelic loss ( FAL ) at 39 autosomal arms also significantly correlated with disease-free survival ( P = 0.013 ) , with an increase in FAL associated with a poorer outcome ; this association remained significant when controlled for tumor thickness ( P = 0.035 ) .
	manualset3
91028	6	399825	5	NULL	NULL	0	NULL	( P = 0.013 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In a subgroup of 41 subjects whose primary tumors were allelotyped , the fractional allelic loss ( FAL ) at 39 autosomal arms also significantly correlated with disease-free survival ( P = 0.013 ) , with an increase in FAL associated with a poorer outcome ; this association remained significant when controlled for tumor thickness ( P = 0.035 ) .
	manualset3
91029	7	399825	5	NULL	NULL	0	NULL	FAL	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a subgroup of 41 subjects whose primary tumors were allelotyped , the fractional allelic loss ( FAL ) at 39 autosomal arms also significantly correlated with disease-free survival ( P = 0.013 ) , with an increase in FAL associated with a poorer outcome ; this association remained significant when controlled for tumor thickness ( P = 0.035 ) .
	manualset3
91030	8	399825	5	NULL	NULL	NULL	NULL	poorer outcome	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a subgroup of 41 subjects whose primary tumors were allelotyped , the fractional allelic loss ( FAL ) at 39 autosomal arms also significantly correlated with disease-free survival ( P = 0.013 ) , with an increase in FAL associated with a poorer outcome ; this association remained significant when controlled for tumor thickness ( P = 0.035 ) .
	manualset3
91031	9	399825	5	NULL	NULL	NULL	NULL	association	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a subgroup of 41 subjects whose primary tumors were allelotyped , the fractional allelic loss ( FAL ) at 39 autosomal arms also significantly correlated with disease-free survival ( P = 0.013 ) , with an increase in FAL associated with a poorer outcome ; this association remained significant when controlled for tumor thickness ( P = 0.035 ) .
	manualset3
91032	10	399825	5	NULL	NULL	0	NULL	tumor thickness ( P = 0.035 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a subgroup of 41 subjects whose primary tumors were allelotyped , the fractional allelic loss ( FAL ) at 39 autosomal arms also significantly correlated with disease-free survival ( P = 0.013 ) , with an increase in FAL associated with a poorer outcome ; this association remained significant when controlled for tumor thickness ( P = 0.035 ) .
	manualset3
91033	1	399826	5	NULL	NULL	0	NULL	time-lagged control design	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a time-lagged control design , six children with migraine headaches were exposed to thermal biofeedback training and then provided performance feedback reflecting moderate and high success , and , if needed , increased feedback frequency .
	manualset3
91034	2	399826	5	NULL	NULL	0	NULL	six children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In a time-lagged control design , six children with migraine headaches were exposed to thermal biofeedback training and then provided performance feedback reflecting moderate and high success , and , if needed , increased feedback frequency .
	manualset3
91035	3	399826	5	NULL	NULL	0	NULL	migraine headaches	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In a time-lagged control design , six children with migraine headaches were exposed to thermal biofeedback training and then provided performance feedback reflecting moderate and high success , and , if needed , increased feedback frequency .
	manualset3
91036	4	399826	5	NULL	NULL	0	NULL	thermal biofeedback training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In a time-lagged control design , six children with migraine headaches were exposed to thermal biofeedback training and then provided performance feedback reflecting moderate and high success , and , if needed , increased feedback frequency .
	manualset3
91037	5	399826	5	NULL	NULL	0	NULL	performance feedback	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In a time-lagged control design , six children with migraine headaches were exposed to thermal biofeedback training and then provided performance feedback reflecting moderate and high success , and , if needed , increased feedback frequency .
	manualset3
91038	6	399826	5	NULL	NULL	0	NULL	moderate and high success	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In a time-lagged control design , six children with migraine headaches were exposed to thermal biofeedback training and then provided performance feedback reflecting moderate and high success , and , if needed , increased feedback frequency .
	manualset3
91039	7	399826	5	NULL	NULL	0	NULL	increased feedback frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a time-lagged control design , six children with migraine headaches were exposed to thermal biofeedback training and then provided performance feedback reflecting moderate and high success , and , if needed , increased feedback frequency .
	manualset3
91040	1	399827	5	NULL	NULL	0	NULL	68 S. Montevideo infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In a total of 68 S. Montevideo infections , 66 cases were contacted .
	manualset3
91041	2	399827	5	NULL	NULL	0	NULL	66 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In a total of 68 S. Montevideo infections , 66 cases were contacted .
	manualset3
91042	1	399828	5	NULL	NULL	0	NULL	transfer test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a transfer test , the dynamic information regarding the displacement of the to-be-moved object could be withdrawn without altering the static visual information that had been available during the learning of the task .
	manualset3
91043	2	399828	5	NULL	NULL	0	NULL	dynamic information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In a transfer test , the dynamic information regarding the displacement of the to-be-moved object could be withdrawn without altering the static visual information that had been available during the learning of the task .
	manualset3
91044	3	399828	5	NULL	NULL	0	NULL	displacement of the to-be-moved object	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In a transfer test , the dynamic information regarding the displacement of the to-be-moved object could be withdrawn without altering the static visual information that had been available during the learning of the task .
	manualset3
91045	4	399828	5	NULL	NULL	0	NULL	static visual information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In a transfer test , the dynamic information regarding the displacement of the to-be-moved object could be withdrawn without altering the static visual information that had been available during the learning of the task .
	manualset3
91046	5	399828	5	NULL	NULL	0	NULL	learning of the task	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In a transfer test , the dynamic information regarding the displacement of the to-be-moved object could be withdrawn without altering the static visual information that had been available during the learning of the task .
	manualset3
91047	1	399829	5	NULL	NULL	0	NULL	transverse retrospective age-adjusted case-control study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a transverse retrospective age-adjusted case-control study , 221 subjects with sinus rhythm without bundle branch block were divided into three groups after signal-averaged ECG acquisition : GI ( N = 40 ) , clinically normal controls , GII ( N = 158 ) , subjects with coronary heart disease without sustained monomorphic ventricular tachycardia ( SMVT ) , and GIII ( N = 23 ) , subjects with heart disease and documented SMVT .
	manualset3
91048	2	399829	5	NULL	NULL	0	NULL	221 subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In a transverse retrospective age-adjusted case-control study , 221 subjects with sinus rhythm without bundle branch block were divided into three groups after signal-averaged ECG acquisition : GI ( N = 40 ) , clinically normal controls , GII ( N = 158 ) , subjects with coronary heart disease without sustained monomorphic ventricular tachycardia ( SMVT ) , and GIII ( N = 23 ) , subjects with heart disease and documented SMVT .
	manualset3
91049	3	399829	5	NULL	NULL	0	NULL	sinus rhythm without bundle branch block	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In a transverse retrospective age-adjusted case-control study , 221 subjects with sinus rhythm without bundle branch block were divided into three groups after signal-averaged ECG acquisition : GI ( N = 40 ) , clinically normal controls , GII ( N = 158 ) , subjects with coronary heart disease without sustained monomorphic ventricular tachycardia ( SMVT ) , and GIII ( N = 23 ) , subjects with heart disease and documented SMVT .
	manualset3
91050	4	399829	5	NULL	NULL	0	NULL	three groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In a transverse retrospective age-adjusted case-control study , 221 subjects with sinus rhythm without bundle branch block were divided into three groups after signal-averaged ECG acquisition : GI ( N = 40 ) , clinically normal controls , GII ( N = 158 ) , subjects with coronary heart disease without sustained monomorphic ventricular tachycardia ( SMVT ) , and GIII ( N = 23 ) , subjects with heart disease and documented SMVT .
	manualset3
91051	5	399829	5	NULL	NULL	0	NULL	signal-averaged ECG acquisition	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In a transverse retrospective age-adjusted case-control study , 221 subjects with sinus rhythm without bundle branch block were divided into three groups after signal-averaged ECG acquisition : GI ( N = 40 ) , clinically normal controls , GII ( N = 158 ) , subjects with coronary heart disease without sustained monomorphic ventricular tachycardia ( SMVT ) , and GIII ( N = 23 ) , subjects with heart disease and documented SMVT .
	manualset3
91052	6	399829	5	NULL	NULL	0	NULL	GI ( N = 40 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In a transverse retrospective age-adjusted case-control study , 221 subjects with sinus rhythm without bundle branch block were divided into three groups after signal-averaged ECG acquisition : GI ( N = 40 ) , clinically normal controls , GII ( N = 158 ) , subjects with coronary heart disease without sustained monomorphic ventricular tachycardia ( SMVT ) , and GIII ( N = 23 ) , subjects with heart disease and documented SMVT .
	manualset3
91053	7	399829	5	NULL	NULL	0	NULL	clinically normal controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In a transverse retrospective age-adjusted case-control study , 221 subjects with sinus rhythm without bundle branch block were divided into three groups after signal-averaged ECG acquisition : GI ( N = 40 ) , clinically normal controls , GII ( N = 158 ) , subjects with coronary heart disease without sustained monomorphic ventricular tachycardia ( SMVT ) , and GIII ( N = 23 ) , subjects with heart disease and documented SMVT .
	manualset3
91054	8	399829	5	NULL	NULL	0	NULL	GII ( N = 158 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In a transverse retrospective age-adjusted case-control study , 221 subjects with sinus rhythm without bundle branch block were divided into three groups after signal-averaged ECG acquisition : GI ( N = 40 ) , clinically normal controls , GII ( N = 158 ) , subjects with coronary heart disease without sustained monomorphic ventricular tachycardia ( SMVT ) , and GIII ( N = 23 ) , subjects with heart disease and documented SMVT .
	manualset3
91055	9	399829	5	NULL	NULL	0	NULL	subjects with coronary heart disease without sustained monomorphic ventricular tachycardia ( SMVT ) , and GIII ( N = 23 )	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In a transverse retrospective age-adjusted case-control study , 221 subjects with sinus rhythm without bundle branch block were divided into three groups after signal-averaged ECG acquisition : GI ( N = 40 ) , clinically normal controls , GII ( N = 158 ) , subjects with coronary heart disease without sustained monomorphic ventricular tachycardia ( SMVT ) , and GIII ( N = 23 ) , subjects with heart disease and documented SMVT .
	manualset3
91056	10	399829	5	NULL	NULL	0	NULL	subjects with heart disease and documented SMVT	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In a transverse retrospective age-adjusted case-control study , 221 subjects with sinus rhythm without bundle branch block were divided into three groups after signal-averaged ECG acquisition : GI ( N = 40 ) , clinically normal controls , GII ( N = 158 ) , subjects with coronary heart disease without sustained monomorphic ventricular tachycardia ( SMVT ) , and GIII ( N = 23 ) , subjects with heart disease and documented SMVT .
	manualset3
91057	1	399830	5	NULL	NULL	0	NULL	 previous analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In accordance with a previous analysis of US cancer mortality , this report also indicates that cancer mortality in the FRG over the last 3 decades ( 1952-1985 ) has not shown any decline commencing in a given period and prevailing in all age groups .
	manualset3
91058	2	399830	5	NULL	NULL	0	NULL	US cancer mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In accordance with a previous analysis of US cancer mortality , this report also indicates that cancer mortality in the FRG over the last 3 decades ( 1952-1985 ) has not shown any decline commencing in a given period and prevailing in all age groups .
	manualset3
91059	3	399830	5	NULL	NULL	0	NULL	report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In accordance with a previous analysis of US cancer mortality , this report also indicates that cancer mortality in the FRG over the last 3 decades ( 1952-1985 ) has not shown any decline commencing in a given period and prevailing in all age groups .
	manualset3
91060	4	399830	5	NULL	NULL	0	NULL	cancer mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In accordance with a previous analysis of US cancer mortality , this report also indicates that cancer mortality in the FRG over the last 3 decades ( 1952-1985 ) has not shown any decline commencing in a given period and prevailing in all age groups .
	manualset3
91061	5	399830	5	NULL	NULL	0	NULL	FRG	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In accordance with a previous analysis of US cancer mortality , this report also indicates that cancer mortality in the FRG over the last 3 decades ( 1952-1985 ) has not shown any decline commencing in a given period and prevailing in all age groups .
	manualset3
91062	6	399830	5	NULL	NULL	0	NULL	over the last 3 decades ( 1952-1985 )	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In accordance with a previous analysis of US cancer mortality , this report also indicates that cancer mortality in the FRG over the last 3 decades ( 1952-1985 ) has not shown any decline commencing in a given period and prevailing in all age groups .
	manualset3
91063	7	399830	5	NULL	NULL	0	NULL	period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In accordance with a previous analysis of US cancer mortality , this report also indicates that cancer mortality in the FRG over the last 3 decades ( 1952-1985 ) has not shown any decline commencing in a given period and prevailing in all age groups .
	manualset3
91064	8	399830	5	NULL	NULL	0	NULL	age groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In accordance with a previous analysis of US cancer mortality , this report also indicates that cancer mortality in the FRG over the last 3 decades ( 1952-1985 ) has not shown any decline commencing in a given period and prevailing in all age groups .
	manualset3
91218	1	399831	5	NULL	NULL	0	NULL	bylaws	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In accordance with the bylaws of the American Psychological Association ( APA ) , the Ethics Committee reports regularly to the membership regarding the number and types of ethics complaints investigated and the major programs undertaken .
	manualset3
91219	2	399831	5	NULL	NULL	0	NULL	American Psychological Association ( APA )	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In accordance with the bylaws of the American Psychological Association ( APA ) , the Ethics Committee reports regularly to the membership regarding the number and types of ethics complaints investigated and the major programs undertaken .
	manualset3
91220	3	399831	5	NULL	NULL	NULL	NULL	Ethics Committee	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In accordance with the bylaws of the American Psychological Association ( APA ) , the Ethics Committee reports regularly to the membership regarding the number and types of ethics complaints investigated and the major programs undertaken .
	manualset3
91221	4	399831	5	NULL	NULL	NULL	NULL	membership	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In accordance with the bylaws of the American Psychological Association ( APA ) , the Ethics Committee reports regularly to the membership regarding the number and types of ethics complaints investigated and the major programs undertaken .
	manualset3
91222	5	399831	5	NULL	NULL	0	NULL	types of ethics complaints	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In accordance with the bylaws of the American Psychological Association ( APA ) , the Ethics Committee reports regularly to the membership regarding the number and types of ethics complaints investigated and the major programs undertaken .
	manualset3
91223	6	399831	5	NULL	NULL	0	NULL	major programs	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In accordance with the bylaws of the American Psychological Association ( APA ) , the Ethics Committee reports regularly to the membership regarding the number and types of ethics complaints investigated and the major programs undertaken .
	manualset3
91224	1	399832	5	NULL	NULL	0	NULL	acute inflammatory effusions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In acute inflammatory effusions their proportion decreased significantly but , as the condition resolved , monocytes began to migrate into the cavity gradually becoming more numerous , transforming into larger macrophages and assuming an increasing phagocytic role .
	manualset3
91225	2	399832	5	NULL	NULL	0	NULL	proportion	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In acute inflammatory effusions their proportion decreased significantly but , as the condition resolved , monocytes began to migrate into the cavity gradually becoming more numerous , transforming into larger macrophages and assuming an increasing phagocytic role .
	manualset3
91226	3	399832	5	NULL	NULL	0	NULL	condition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In acute inflammatory effusions their proportion decreased significantly but , as the condition resolved , monocytes began to migrate into the cavity gradually becoming more numerous , transforming into larger macrophages and assuming an increasing phagocytic role .
	manualset3
91227	4	399832	5	NULL	NULL	0	NULL	monocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In acute inflammatory effusions their proportion decreased significantly but , as the condition resolved , monocytes began to migrate into the cavity gradually becoming more numerous , transforming into larger macrophages and assuming an increasing phagocytic role .
	manualset3
91228	5	399832	5	NULL	NULL	0	NULL	cavity	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In acute inflammatory effusions their proportion decreased significantly but , as the condition resolved , monocytes began to migrate into the cavity gradually becoming more numerous , transforming into larger macrophages and assuming an increasing phagocytic role .
	manualset3
91229	6	399832	5	NULL	NULL	0	NULL	larger macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In acute inflammatory effusions their proportion decreased significantly but , as the condition resolved , monocytes began to migrate into the cavity gradually becoming more numerous , transforming into larger macrophages and assuming an increasing phagocytic role .
	manualset3
91230	7	399832	5	NULL	NULL	0	NULL	phagocytic role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In acute inflammatory effusions their proportion decreased significantly but , as the condition resolved , monocytes began to migrate into the cavity gradually becoming more numerous , transforming into larger macrophages and assuming an increasing phagocytic role .
	manualset3
91231	1	399833	5	NULL	NULL	0	NULL	( NH 4 ) 5 { Hf ( PMo 12O 40 ) ( ( NH 4 ) PMo 11O 39 ) } .23.5 H 2O	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , ( NH 4 ) 5 { Hf ( PMo 12O 40 ) ( ( NH 4 ) PMo 11O 39 ) } .23.5 H 2O can be crystallized as a minor product .
	manualset3
91232	2	399833	5	NULL	NULL	0	NULL	minor product	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , ( NH 4 ) 5 { Hf ( PMo 12O 40 ) ( ( NH 4 ) PMo 11O 39 ) } .23.5 H 2O can be crystallized as a minor product .
	manualset3
91233	1	399834	5	NULL	NULL	0	NULL	110 ( 6 ) bone marrow ( BM ) cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , 110 ( 6 ) bone marrow ( BM ) cells were injected into five locations in the ischemic muscle immediately after ligation and artery excision .
	manualset3
91234	2	399834	5	NULL	NULL	NULL	NULL	five locations	AnatomicalPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , 110 ( 6 ) bone marrow ( BM ) cells were injected into five locations in the ischemic muscle immediately after ligation and artery excision .
	manualset3
91235	3	399834	5	NULL	NULL	0	NULL	ischemic muscle	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , 110 ( 6 ) bone marrow ( BM ) cells were injected into five locations in the ischemic muscle immediately after ligation and artery excision .
	manualset3
91236	4	399834	5	NULL	NULL	0	NULL	ligation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , 110 ( 6 ) bone marrow ( BM ) cells were injected into five locations in the ischemic muscle immediately after ligation and artery excision .
	manualset3
91237	5	399834	5	NULL	NULL	0	NULL	artery excision	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , 110 ( 6 ) bone marrow ( BM ) cells were injected into five locations in the ischemic muscle immediately after ligation and artery excision .
	manualset3
91238	1	399835	5	NULL	NULL	0	NULL	40 excited states of the complex	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , 40 excited states of the complex were calculated and assigned symmetry based on a C ( 2v ) symmetry of the optimized complex found with B3LYP/LANL2DZ .
	manualset3
91819	2	399835	5	NULL	NULL	0	NULL	symmetry	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , 40 excited states of the complex were calculated and assigned symmetry based on a C ( 2v ) symmetry of the optimized complex found with B3LYP/LANL2DZ .
	manualset3
91820	3	399835	5	NULL	NULL	0	NULL	C ( 2v ) symmetry	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , 40 excited states of the complex were calculated and assigned symmetry based on a C ( 2v ) symmetry of the optimized complex found with B3LYP/LANL2DZ .
	manualset3
91821	4	399835	5	NULL	NULL	0	NULL	optimized complex	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , 40 excited states of the complex were calculated and assigned symmetry based on a C ( 2v ) symmetry of the optimized complex found with B3LYP/LANL2DZ .
	manualset3
91822	5	399835	5	NULL	NULL	0	NULL	B3LYP/LANL2DZ	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , 40 excited states of the complex were calculated and assigned symmetry based on a C ( 2v ) symmetry of the optimized complex found with B3LYP/LANL2DZ .
	manualset3
91825	1	399836	5	NULL	NULL	NULL	NULL	AD4743	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , AD4743 ( 1-10 micrograms/ml ) in the presence of 25 % HP markedly increased the kinetics of adipocyte differentiation , at low ( less than 5 , 000 cells/cm2 ) or high cell density .
	manualset3
91828	2	399836	5	NULL	NULL	0	NULL	25 % HP	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , AD4743 ( 1-10 micrograms/ml ) in the presence of 25 % HP markedly increased the kinetics of adipocyte differentiation , at low ( less than 5 , 000 cells/cm2 ) or high cell density .
	manualset3
91829	3	399836	5	NULL	NULL	0	NULL	adipocyte differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , AD4743 ( 1-10 micrograms/ml ) in the presence of 25 % HP markedly increased the kinetics of adipocyte differentiation , at low ( less than 5 , 000 cells/cm2 ) or high cell density .
	manualset3
91831	4	399836	5	NULL	NULL	0	NULL	less than 5 , 000 cells/cm2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , AD4743 ( 1-10 micrograms/ml ) in the presence of 25 % HP markedly increased the kinetics of adipocyte differentiation , at low ( less than 5 , 000 cells/cm2 ) or high cell density .
	manualset3
91833	5	399836	5	NULL	NULL	0	NULL	high cell density	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , AD4743 ( 1-10 micrograms/ml ) in the presence of 25 % HP markedly increased the kinetics of adipocyte differentiation , at low ( less than 5 , 000 cells/cm2 ) or high cell density .
	manualset3
93336	6	399836	5	NULL	NULL	0	NULL	1-10 micrograms/ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , AD4743 ( 1-10 micrograms/ml ) in the presence of 25 % HP markedly increased the kinetics of adipocyte differentiation , at low ( less than 5 , 000 cells/cm2 ) or high cell density .
	manualset3
91835	1	399837	5	NULL	NULL	0	NULL	Beclin-1 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , Beclin-1 expression after injury is elevated also in astrocytes starting at 3 days after injury .
	manualset3
91837	2	399837	5	NULL	NULL	0	NULL	injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , Beclin-1 expression after injury is elevated also in astrocytes starting at 3 days after injury .
	manualset3
91838	3	399837	5	NULL	NULL	0	NULL	astrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , Beclin-1 expression after injury is elevated also in astrocytes starting at 3 days after injury .
	manualset3
91840	4	399837	5	NULL	NULL	0	NULL	3 days after injury	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , Beclin-1 expression after injury is elevated also in astrocytes starting at 3 days after injury .
	manualset3
91853	1	399838	5	NULL	NULL	0	NULL	EOP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , EOP did not follow the same time-course of other physiological adaptations as no differences ( day 1 vs. 4 vs. 8 ) in resting or exercise levels were observed over the eight day heat acclimation regime .
	manualset3
91854	2	399838	5	NULL	NULL	0	NULL	time-course	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , EOP did not follow the same time-course of other physiological adaptations as no differences ( day 1 vs. 4 vs. 8 ) in resting or exercise levels were observed over the eight day heat acclimation regime .
	manualset3
91858	3	399838	5	NULL	NULL	0	NULL	physiological adaptations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , EOP did not follow the same time-course of other physiological adaptations as no differences ( day 1 vs. 4 vs. 8 ) in resting or exercise levels were observed over the eight day heat acclimation regime .
	manualset3
91859	4	399838	5	NULL	NULL	NULL	NULL	day 1 vs. 4 vs. 8	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , EOP did not follow the same time-course of other physiological adaptations as no differences ( day 1 vs. 4 vs. 8 ) in resting or exercise levels were observed over the eight day heat acclimation regime .
	manualset3
91862	5	399838	5	NULL	NULL	0	NULL	resting or exercise levels 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , EOP did not follow the same time-course of other physiological adaptations as no differences ( day 1 vs. 4 vs. 8 ) in resting or exercise levels were observed over the eight day heat acclimation regime .
	manualset3
91866	6	399838	5	NULL	NULL	NULL	NULL	eight day heat acclimation regime	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , EOP did not follow the same time-course of other physiological adaptations as no differences ( day 1 vs. 4 vs. 8 ) in resting or exercise levels were observed over the eight day heat acclimation regime .
	manualset3
91876	1	399839	5	NULL	NULL	0	NULL	Upper fibroscopy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Upper fibroscopy and enteromesenteric infarction ) .
	manualset3
91878	2	399839	5	NULL	NULL	0	NULL	enteromesenteric infarction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Upper fibroscopy and enteromesenteric infarction ) .
	manualset3
91879	1	399840	5	NULL	NULL	0	NULL	Fos-ir neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , Fos-ir neurons were evident after NGF administration in areas devoid of immunopositive cells in control animals .
	manualset3
91880	2	399840	5	NULL	NULL	0	NULL	NGF administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , Fos-ir neurons were evident after NGF administration in areas devoid of immunopositive cells in control animals .
	manualset3
91881	3	399840	5	NULL	NULL	0	NULL	areas devoid of immunopositive cells	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , Fos-ir neurons were evident after NGF administration in areas devoid of immunopositive cells in control animals .
	manualset3
91882	4	399840	5	NULL	NULL	0	NULL	control animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , Fos-ir neurons were evident after NGF administration in areas devoid of immunopositive cells in control animals .
	manualset3
91883	1	399841	5	NULL	NULL	0	NULL	GnRH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , GnRH suppressed FSH-stimulated LH receptor mRNA levels in a dose-dependent manner ; the effects of GnRH could be counteracted by coincubation with a GnRH antagonist , suggesting mediation by specific GnRH-binding sites .
	manualset3
91884	2	399841	5	NULL	NULL	0	NULL	FSH-stimulated LH receptor mRNA levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , GnRH suppressed FSH-stimulated LH receptor mRNA levels in a dose-dependent manner ; the effects of GnRH could be counteracted by coincubation with a GnRH antagonist , suggesting mediation by specific GnRH-binding sites .
	manualset3
91885	3	399841	5	NULL	NULL	NULL	NULL	effects of GnRH	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , GnRH suppressed FSH-stimulated LH receptor mRNA levels in a dose-dependent manner ; the effects of GnRH could be counteracted by coincubation with a GnRH antagonist , suggesting mediation by specific GnRH-binding sites .
	manualset3
91886	4	399841	5	NULL	NULL	0	NULL	coincubation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , GnRH suppressed FSH-stimulated LH receptor mRNA levels in a dose-dependent manner ; the effects of GnRH could be counteracted by coincubation with a GnRH antagonist , suggesting mediation by specific GnRH-binding sites .
	manualset3
91887	5	399841	5	NULL	NULL	0	NULL	GnRH antagonist	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , GnRH suppressed FSH-stimulated LH receptor mRNA levels in a dose-dependent manner ; the effects of GnRH could be counteracted by coincubation with a GnRH antagonist , suggesting mediation by specific GnRH-binding sites .
	manualset3
91888	6	399841	5	NULL	NULL	NULL	NULL	mediation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , GnRH suppressed FSH-stimulated LH receptor mRNA levels in a dose-dependent manner ; the effects of GnRH could be counteracted by coincubation with a GnRH antagonist , suggesting mediation by specific GnRH-binding sites .
	manualset3
91889	7	399841	5	NULL	NULL	0	NULL	GnRH-binding sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , GnRH suppressed FSH-stimulated LH receptor mRNA levels in a dose-dependent manner ; the effects of GnRH could be counteracted by coincubation with a GnRH antagonist , suggesting mediation by specific GnRH-binding sites .
	manualset3
91890	1	399842	5	NULL	NULL	0	NULL	IGF-I-dependent MAPK activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , IGF-I-dependent MAPK activation was also impaired , and SMC proliferation in response to IGF-I was inhibited .
	manualset3
91891	2	399842	5	NULL	NULL	NULL	NULL	SMC proliferation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , IGF-I-dependent MAPK activation was also impaired , and SMC proliferation in response to IGF-I was inhibited .
	manualset3
91892	3	399842	5	NULL	NULL	0	NULL	IGF-I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , IGF-I-dependent MAPK activation was also impaired , and SMC proliferation in response to IGF-I was inhibited .
	manualset3
91893	1	399843	5	NULL	NULL	0	NULL	IL-10-stimulated monocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , IL-10-stimulated monocytes are more efficiently infected by HIV BaL .
	manualset3
91894	2	399843	5	NULL	NULL	0	NULL	HIV BaL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , IL-10-stimulated monocytes are more efficiently infected by HIV BaL .
	manualset3
91925	1	399844	5	NULL	NULL	0	NULL	MD simulations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , MD simulations allowed the analysis of the stability of tetrameric MtCDA structure .
	manualset3
91928	2	399844	5	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , MD simulations allowed the analysis of the stability of tetrameric MtCDA structure .
	manualset3
91930	3	399844	5	NULL	NULL	0	NULL	tetrameric MtCDA structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , MD simulations allowed the analysis of the stability of tetrameric MtCDA structure .
	manualset3
91953	1	399845	5	NULL	NULL	0	NULL	 MMP-2 inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , MMP-2 inhibition in the tumor cells decreased the expression of stromal cell-derived factor 1 ( SDF1 ) in the tumor-conditioned medium , which results in impaired SDF1/CXCR4 signaling leading to decreased stem cell tropism towards the tumor cells .
	manualset3
91954	2	399845	5	NULL	NULL	0	NULL	tumor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , MMP-2 inhibition in the tumor cells decreased the expression of stromal cell-derived factor 1 ( SDF1 ) in the tumor-conditioned medium , which results in impaired SDF1/CXCR4 signaling leading to decreased stem cell tropism towards the tumor cells .
	manualset3
91955	3	399845	5	NULL	NULL	0	NULL	expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , MMP-2 inhibition in the tumor cells decreased the expression of stromal cell-derived factor 1 ( SDF1 ) in the tumor-conditioned medium , which results in impaired SDF1/CXCR4 signaling leading to decreased stem cell tropism towards the tumor cells .
	manualset3
91956	4	399845	5	NULL	NULL	0	NULL	stromal cell-derived factor 1 ( SDF1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , MMP-2 inhibition in the tumor cells decreased the expression of stromal cell-derived factor 1 ( SDF1 ) in the tumor-conditioned medium , which results in impaired SDF1/CXCR4 signaling leading to decreased stem cell tropism towards the tumor cells .
	manualset3
91957	5	399845	5	NULL	NULL	0	NULL	tumor-conditioned medium	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , MMP-2 inhibition in the tumor cells decreased the expression of stromal cell-derived factor 1 ( SDF1 ) in the tumor-conditioned medium , which results in impaired SDF1/CXCR4 signaling leading to decreased stem cell tropism towards the tumor cells .
	manualset3
91958	6	399845	5	NULL	NULL	0	NULL	impaired SDF1/CXCR4 signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , MMP-2 inhibition in the tumor cells decreased the expression of stromal cell-derived factor 1 ( SDF1 ) in the tumor-conditioned medium , which results in impaired SDF1/CXCR4 signaling leading to decreased stem cell tropism towards the tumor cells .
	manualset3
91962	7	399845	5	NULL	NULL	0	NULL	decreased stem cell tropism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , MMP-2 inhibition in the tumor cells decreased the expression of stromal cell-derived factor 1 ( SDF1 ) in the tumor-conditioned medium , which results in impaired SDF1/CXCR4 signaling leading to decreased stem cell tropism towards the tumor cells .
	manualset3
91963	8	399845	5	NULL	NULL	0	NULL	tumor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , MMP-2 inhibition in the tumor cells decreased the expression of stromal cell-derived factor 1 ( SDF1 ) in the tumor-conditioned medium , which results in impaired SDF1/CXCR4 signaling leading to decreased stem cell tropism towards the tumor cells .
	manualset3
92131	1	399846	5	NULL	NULL	0	NULL	Monoclea	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , Monoclea was found to have branched plasmodesmata , and plasmodesmata of Sphagnum displayed densely staining regions around the neck region , as well as ring-like wall specializations .
	manualset3
92132	2	399846	5	NULL	NULL	0	NULL	branched plasmodesmata	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , Monoclea was found to have branched plasmodesmata , and plasmodesmata of Sphagnum displayed densely staining regions around the neck region , as well as ring-like wall specializations .
	manualset3
92133	3	399846	5	NULL	NULL	0	NULL	plasmodesmata	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , Monoclea was found to have branched plasmodesmata , and plasmodesmata of Sphagnum displayed densely staining regions around the neck region , as well as ring-like wall specializations .
	manualset3
92134	4	399846	5	NULL	NULL	0	NULL	Sphagnum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , Monoclea was found to have branched plasmodesmata , and plasmodesmata of Sphagnum displayed densely staining regions around the neck region , as well as ring-like wall specializations .
	manualset3
92135	5	399846	5	NULL	NULL	NULL	NULL	densely staining regions around the neck region	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , Monoclea was found to have branched plasmodesmata , and plasmodesmata of Sphagnum displayed densely staining regions around the neck region , as well as ring-like wall specializations .
	manualset3
92136	6	399846	5	NULL	NULL	0	NULL	ring-like wall specializations	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , Monoclea was found to have branched plasmodesmata , and plasmodesmata of Sphagnum displayed densely staining regions around the neck region , as well as ring-like wall specializations .
	manualset3
92137	1	399847	5	NULL	NULL	0	NULL	PI 3-K	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , PI 3-K is involved in the activation of the Ras-ERK pathway in human HSC , although it is not strictly necessary , since established PI 3-K inhibitors inhibit ERK activation only by 40-50 % .
	manualset3
92138	2	399847	5	NULL	NULL	0	NULL	activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , PI 3-K is involved in the activation of the Ras-ERK pathway in human HSC , although it is not strictly necessary , since established PI 3-K inhibitors inhibit ERK activation only by 40-50 % .
	manualset3
92139	3	399847	5	NULL	NULL	0	NULL	Ras-ERK pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , PI 3-K is involved in the activation of the Ras-ERK pathway in human HSC , although it is not strictly necessary , since established PI 3-K inhibitors inhibit ERK activation only by 40-50 % .
	manualset3
92140	4	399847	5	NULL	NULL	0	NULL	human HSC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , PI 3-K is involved in the activation of the Ras-ERK pathway in human HSC , although it is not strictly necessary , since established PI 3-K inhibitors inhibit ERK activation only by 40-50 % .
	manualset3
92141	5	399847	5	NULL	NULL	0	NULL	established PI 3-K inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , PI 3-K is involved in the activation of the Ras-ERK pathway in human HSC , although it is not strictly necessary , since established PI 3-K inhibitors inhibit ERK activation only by 40-50 % .
	manualset3
92142	6	399847	5	NULL	NULL	0	NULL	ERK activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , PI 3-K is involved in the activation of the Ras-ERK pathway in human HSC , although it is not strictly necessary , since established PI 3-K inhibitors inhibit ERK activation only by 40-50 % .
	manualset3
92143	7	399847	5	NULL	NULL	0	NULL	40-50 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , PI 3-K is involved in the activation of the Ras-ERK pathway in human HSC , although it is not strictly necessary , since established PI 3-K inhibitors inhibit ERK activation only by 40-50 % .
	manualset3
92144	1	399848	5	NULL	NULL	0	NULL	PVAE	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , PVAE attenuated phorbol 12-myristate 13-acetate ( PMA ) and calcium ionophore A23187-stimulated TNF-alpha , IL-6 , and IL-8 secretion in human mast cells .
	manualset3
92145	2	399848	5	NULL	NULL	0	NULL	phorbol 12-myristate 13-acetate ( PMA ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , PVAE attenuated phorbol 12-myristate 13-acetate ( PMA ) and calcium ionophore A23187-stimulated TNF-alpha , IL-6 , and IL-8 secretion in human mast cells .
	manualset3
92146	3	399848	5	NULL	NULL	0	NULL	calcium ionophore A23187-stimulated TNF-alpha secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , PVAE attenuated phorbol 12-myristate 13-acetate ( PMA ) and calcium ionophore A23187-stimulated TNF-alpha , IL-6 , and IL-8 secretion in human mast cells .
	manualset3
92147	4	399848	5	NULL	NULL	0	NULL	calcium ionophore A23187-stimulated IL-6 secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , PVAE attenuated phorbol 12-myristate 13-acetate ( PMA ) and calcium ionophore A23187-stimulated TNF-alpha , IL-6 , and IL-8 secretion in human mast cells .
	manualset3
92148	5	399848	5	NULL	NULL	0	NULL	calcium ionophore A23187-stimulated IL-8 secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , PVAE attenuated phorbol 12-myristate 13-acetate ( PMA ) and calcium ionophore A23187-stimulated TNF-alpha , IL-6 , and IL-8 secretion in human mast cells .
	manualset3
92149	6	399848	5	NULL	NULL	0	NULL	human mast cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , PVAE attenuated phorbol 12-myristate 13-acetate ( PMA ) and calcium ionophore A23187-stimulated TNF-alpha , IL-6 , and IL-8 secretion in human mast cells .
	manualset3
92150	1	399849	5	NULL	NULL	0	NULL	REFs transfected with E1A - but not core-expressing plasmid	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , REFs transfected with E1A - but not core-expressing plasmid showed the phenotype of immortalized cells when selected with G418 .
	manualset3
92151	2	399849	5	NULL	NULL	0	NULL	phenotype	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , REFs transfected with E1A - but not core-expressing plasmid showed the phenotype of immortalized cells when selected with G418 .
	manualset3
92152	3	399849	5	NULL	NULL	0	NULL	immortalized cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , REFs transfected with E1A - but not core-expressing plasmid showed the phenotype of immortalized cells when selected with G418 .
	manualset3
92153	4	399849	5	NULL	NULL	0	NULL	G418	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , REFs transfected with E1A - but not core-expressing plasmid showed the phenotype of immortalized cells when selected with G418 .
	manualset3
92154	1	399850	5	NULL	NULL	NULL	NULL	SHM	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , SHM was skewed toward transitions at G/C residues .
	manualset3
92155	2	399850	5	NULL	NULL	0	NULL	transitions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , SHM was skewed toward transitions at G/C residues .
	manualset3
92156	3	399850	5	NULL	NULL	0	NULL	G/C residues	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , SHM was skewed toward transitions at G/C residues .
	manualset3
92157	1	399851	5	NULL	NULL	0	NULL	StCO	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , StCO affected the mRNA levels of StBEL5 - a tuberization promoter , the mRNA of which moves long distances in potato plants - and StFT/StSP6A , a protein highly similar to FLOWERING LOCUST ( FT ) , which is a key component of systemic flowering signals in other species .
	manualset3
92158	2	399851	5	NULL	NULL	0	NULL	mRNA levels	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , StCO affected the mRNA levels of StBEL5 - a tuberization promoter , the mRNA of which moves long distances in potato plants - and StFT/StSP6A , a protein highly similar to FLOWERING LOCUST ( FT ) , which is a key component of systemic flowering signals in other species .
	manualset3
92159	3	399851	5	NULL	NULL	NULL	NULL	StBEL5 - a tuberization promoter	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , StCO affected the mRNA levels of StBEL5 - a tuberization promoter , the mRNA of which moves long distances in potato plants - and StFT/StSP6A , a protein highly similar to FLOWERING LOCUST ( FT ) , which is a key component of systemic flowering signals in other species .
	manualset3
92160	4	399851	5	NULL	NULL	0	NULL	StBEL5 - a tuberization promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , StCO affected the mRNA levels of StBEL5 - a tuberization promoter , the mRNA of which moves long distances in potato plants - and StFT/StSP6A , a protein highly similar to FLOWERING LOCUST ( FT ) , which is a key component of systemic flowering signals in other species .
	manualset3
92161	5	399851	5	NULL	NULL	0	NULL	mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , StCO affected the mRNA levels of StBEL5 - a tuberization promoter , the mRNA of which moves long distances in potato plants - and StFT/StSP6A , a protein highly similar to FLOWERING LOCUST ( FT ) , which is a key component of systemic flowering signals in other species .
	manualset3
92162	6	399851	5	NULL	NULL	0	NULL	long distances	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , StCO affected the mRNA levels of StBEL5 - a tuberization promoter , the mRNA of which moves long distances in potato plants - and StFT/StSP6A , a protein highly similar to FLOWERING LOCUST ( FT ) , which is a key component of systemic flowering signals in other species .
	manualset3
92163	7	399851	5	NULL	NULL	0	NULL	potato plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , StCO affected the mRNA levels of StBEL5 - a tuberization promoter , the mRNA of which moves long distances in potato plants - and StFT/StSP6A , a protein highly similar to FLOWERING LOCUST ( FT ) , which is a key component of systemic flowering signals in other species .
	manualset3
92164	8	399851	5	NULL	NULL	0	NULL	StFT/StSP6A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , StCO affected the mRNA levels of StBEL5 - a tuberization promoter , the mRNA of which moves long distances in potato plants - and StFT/StSP6A , a protein highly similar to FLOWERING LOCUST ( FT ) , which is a key component of systemic flowering signals in other species .
	manualset3
92165	9	399851	5	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , StCO affected the mRNA levels of StBEL5 - a tuberization promoter , the mRNA of which moves long distances in potato plants - and StFT/StSP6A , a protein highly similar to FLOWERING LOCUST ( FT ) , which is a key component of systemic flowering signals in other species .
	manualset3
92166	10	399851	5	NULL	NULL	0	NULL	FLOWERING LOCUST ( FT ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , StCO affected the mRNA levels of StBEL5 - a tuberization promoter , the mRNA of which moves long distances in potato plants - and StFT/StSP6A , a protein highly similar to FLOWERING LOCUST ( FT ) , which is a key component of systemic flowering signals in other species .
	manualset3
92167	11	399851	5	NULL	NULL	0	NULL	key component	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , StCO affected the mRNA levels of StBEL5 - a tuberization promoter , the mRNA of which moves long distances in potato plants - and StFT/StSP6A , a protein highly similar to FLOWERING LOCUST ( FT ) , which is a key component of systemic flowering signals in other species .
	manualset3
92168	12	399851	5	NULL	NULL	0	NULL	systemic flowering signals	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , StCO affected the mRNA levels of StBEL5 - a tuberization promoter , the mRNA of which moves long distances in potato plants - and StFT/StSP6A , a protein highly similar to FLOWERING LOCUST ( FT ) , which is a key component of systemic flowering signals in other species .
	manualset3
92169	13	399851	5	NULL	NULL	0	NULL	other species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , StCO affected the mRNA levels of StBEL5 - a tuberization promoter , the mRNA of which moves long distances in potato plants - and StFT/StSP6A , a protein highly similar to FLOWERING LOCUST ( FT ) , which is a key component of systemic flowering signals in other species .
	manualset3
92170	1	399852	5	NULL	NULL	0	NULL	T3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , T3 increases mitochondrial TFA expression , a mitochondrial transcription factor encoded by a nuclear gene .
	manualset3
92171	2	399852	5	NULL	NULL	0	NULL	mitochondrial TFA expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , T3 increases mitochondrial TFA expression , a mitochondrial transcription factor encoded by a nuclear gene .
	manualset3
92172	3	399852	5	NULL	NULL	0	NULL	mitochondrial transcription factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , T3 increases mitochondrial TFA expression , a mitochondrial transcription factor encoded by a nuclear gene .
	manualset3
92173	4	399852	5	NULL	NULL	0	NULL	nuclear gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , T3 increases mitochondrial TFA expression , a mitochondrial transcription factor encoded by a nuclear gene .
	manualset3
92174	1	399853	5	NULL	NULL	0	NULL	Thy-B lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , Thy-B lymphocytes showed peculiar patterns both of adhesion molecules ( CD62L ( - ) , CD44 ( intermediate ) ) , and of activation molecules ( CD69 ( + ) , CD80 ( + ) , and , in part , CD95 ( + ) ) .
	manualset3
92175	2	399853	5	NULL	NULL	0	NULL	adhesion molecules ( CD62L ( - ) , CD44 ( intermediate ) )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , Thy-B lymphocytes showed peculiar patterns both of adhesion molecules ( CD62L ( - ) , CD44 ( intermediate ) ) , and of activation molecules ( CD69 ( + ) , CD80 ( + ) , and , in part , CD95 ( + ) ) .
	manualset3
92176	3	399853	5	NULL	NULL	0	NULL	activation molecules ( CD69 ( + ) , CD80 ( + ) , and , in part , CD95 ( + ) )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , Thy-B lymphocytes showed peculiar patterns both of adhesion molecules ( CD62L ( - ) , CD44 ( intermediate ) ) , and of activation molecules ( CD69 ( + ) , CD80 ( + ) , and , in part , CD95 ( + ) ) .
	manualset3
92177	1	399854	5	NULL	NULL	0	NULL	2-kb segment upstream of the epsilon-globin gene	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , a 2-kb segment upstream of the epsilon-globin gene was sequenced in two of the five strepsirhines examined .
	manualset3
92178	2	399854	5	NULL	NULL	0	NULL	strepsirhines	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , a 2-kb segment upstream of the epsilon-globin gene was sequenced in two of the five strepsirhines examined .
	manualset3
92179	1	399855	5	NULL	NULL	NULL	NULL	HindIII digest of lambda	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , a HindIII digest of lambda was present in a separate lane in each run .
	manualset3
92181	2	399855	5	NULL	NULL	0	NULL	separate lane	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , a HindIII digest of lambda was present in a separate lane in each run .
	manualset3
92182	1	399856	5	NULL	NULL	0	NULL	 commercial IgG fraction	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , a commercial IgG fraction from mouse plasma similarly labeled the Golgi area , unlike IgG from mouse serum from another source .
	manualset3
92183	2	399856	5	NULL	NULL	0	NULL	mouse plasma	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , a commercial IgG fraction from mouse plasma similarly labeled the Golgi area , unlike IgG from mouse serum from another source .
	manualset3
92184	3	399856	5	NULL	NULL	0	NULL	Golgi area	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , a commercial IgG fraction from mouse plasma similarly labeled the Golgi area , unlike IgG from mouse serum from another source .
	manualset3
92185	4	399856	5	NULL	NULL	0	NULL	IgG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , a commercial IgG fraction from mouse plasma similarly labeled the Golgi area , unlike IgG from mouse serum from another source .
	manualset3
92186	5	399856	5	NULL	NULL	0	NULL	mouse serum	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , a commercial IgG fraction from mouse plasma similarly labeled the Golgi area , unlike IgG from mouse serum from another source .
	manualset3
92187	6	399856	5	NULL	NULL	0	NULL	another source	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , a commercial IgG fraction from mouse plasma similarly labeled the Golgi area , unlike IgG from mouse serum from another source .
	manualset3
92188	1	399857	5	NULL	NULL	0	NULL	dynamic ( steady-state ) flux model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , a dynamic ( steady-state ) flux model for uptake with transpiration water into thick roots is presented .
	manualset3
92189	2	399857	5	NULL	NULL	0	NULL	uptake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , a dynamic ( steady-state ) flux model for uptake with transpiration water into thick roots is presented .
	manualset3
92190	3	399857	5	NULL	NULL	0	NULL	transpiration water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , a dynamic ( steady-state ) flux model for uptake with transpiration water into thick roots is presented .
	manualset3
92191	4	399857	5	NULL	NULL	0	NULL	thick roots	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , a dynamic ( steady-state ) flux model for uptake with transpiration water into thick roots is presented .
	manualset3
92192	1	399858	5	NULL	NULL	0	NULL	adrenergic beta blockaders	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Use of adrenergic beta blockaders in thyrotoxicosis and hypothyroidism ) .
	manualset3
92193	2	399858	5	NULL	NULL	0	NULL	thyrotoxicosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Use of adrenergic beta blockaders in thyrotoxicosis and hypothyroidism ) .
	manualset3
92194	3	399858	5	NULL	NULL	0	NULL	hypothyroidism	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Use of adrenergic beta blockaders in thyrotoxicosis and hypothyroidism ) .
	manualset3
92195	1	399859	5	NULL	NULL	0	NULL	laser measurement system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , a laser measurement system was developed to confirm the induced strain in the samples .
	manualset3
92196	2	399859	5	NULL	NULL	NULL	NULL	strain	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , a laser measurement system was developed to confirm the induced strain in the samples .
	manualset3
92197	3	399859	5	NULL	NULL	0	NULL	samples	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , a laser measurement system was developed to confirm the induced strain in the samples .
	manualset3
92198	1	399860	5	NULL	NULL	0	NULL	petrol vapor	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , a single attempt to ignite petrol vapor emanating from a pool of liquid fuel was effected with a smouldering piece of cannabis resin ; no ignition occurred .
	manualset3
92199	2	399860	5	NULL	NULL	0	NULL	pool of liquid fuel	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , a single attempt to ignite petrol vapor emanating from a pool of liquid fuel was effected with a smouldering piece of cannabis resin ; no ignition occurred .
	manualset3
92200	3	399860	5	NULL	NULL	NULL	NULL	smouldering piece of cannabis resin	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , a single attempt to ignite petrol vapor emanating from a pool of liquid fuel was effected with a smouldering piece of cannabis resin ; no ignition occurred .
	manualset3
92201	4	399860	5	NULL	NULL	0	NULL	ignition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , a single attempt to ignite petrol vapor emanating from a pool of liquid fuel was effected with a smouldering piece of cannabis resin ; no ignition occurred .
	manualset3
92202	1	399861	5	NULL	NULL	NULL	NULL	acetylbergenin	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , acetylbergenin doses of 50 mg/kg showed almost the same levels of hepatoprotective activity as 100 mg/kg of bergenin , indicating that lipophilic acetylbergenin is more active against the antihepatotoxic effects of CCl4 than those of the much less lipophilic bergenin .
	manualset3
92203	2	399861	5	NULL	NULL	0	NULL	levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , acetylbergenin doses of 50 mg/kg showed almost the same levels of hepatoprotective activity as 100 mg/kg of bergenin , indicating that lipophilic acetylbergenin is more active against the antihepatotoxic effects of CCl4 than those of the much less lipophilic bergenin .
	manualset3
92204	3	399861	5	NULL	NULL	0	NULL	hepatoprotective activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , acetylbergenin doses of 50 mg/kg showed almost the same levels of hepatoprotective activity as 100 mg/kg of bergenin , indicating that lipophilic acetylbergenin is more active against the antihepatotoxic effects of CCl4 than those of the much less lipophilic bergenin .
	manualset3
92205	4	399861	5	NULL	NULL	NULL	NULL	100 mg/kg	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , acetylbergenin doses of 50 mg/kg showed almost the same levels of hepatoprotective activity as 100 mg/kg of bergenin , indicating that lipophilic acetylbergenin is more active against the antihepatotoxic effects of CCl4 than those of the much less lipophilic bergenin .
	manualset3
92206	5	399861	5	NULL	NULL	0	NULL	lipophilic acetylbergenin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , acetylbergenin doses of 50 mg/kg showed almost the same levels of hepatoprotective activity as 100 mg/kg of bergenin , indicating that lipophilic acetylbergenin is more active against the antihepatotoxic effects of CCl4 than those of the much less lipophilic bergenin .
	manualset3
92207	6	399861	5	NULL	NULL	0	NULL	antihepatotoxic effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , acetylbergenin doses of 50 mg/kg showed almost the same levels of hepatoprotective activity as 100 mg/kg of bergenin , indicating that lipophilic acetylbergenin is more active against the antihepatotoxic effects of CCl4 than those of the much less lipophilic bergenin .
	manualset3
92208	7	399861	5	NULL	NULL	0	NULL	CCl4	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , acetylbergenin doses of 50 mg/kg showed almost the same levels of hepatoprotective activity as 100 mg/kg of bergenin , indicating that lipophilic acetylbergenin is more active against the antihepatotoxic effects of CCl4 than those of the much less lipophilic bergenin .
	manualset3
92209	8	399861	5	NULL	NULL	0	NULL	lipophilic bergenin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , acetylbergenin doses of 50 mg/kg showed almost the same levels of hepatoprotective activity as 100 mg/kg of bergenin , indicating that lipophilic acetylbergenin is more active against the antihepatotoxic effects of CCl4 than those of the much less lipophilic bergenin .
	manualset3
93337	9	399861	5	NULL	NULL	0	NULL	doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , acetylbergenin doses of 50 mg/kg showed almost the same levels of hepatoprotective activity as 100 mg/kg of bergenin , indicating that lipophilic acetylbergenin is more active against the antihepatotoxic effects of CCl4 than those of the much less lipophilic bergenin .
	manualset3
93338	10	399861	5	NULL	NULL	0	NULL	50 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , acetylbergenin doses of 50 mg/kg showed almost the same levels of hepatoprotective activity as 100 mg/kg of bergenin , indicating that lipophilic acetylbergenin is more active against the antihepatotoxic effects of CCl4 than those of the much less lipophilic bergenin .
	manualset3
93339	11	399861	5	NULL	NULL	0	NULL	bergenin	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , acetylbergenin doses of 50 mg/kg showed almost the same levels of hepatoprotective activity as 100 mg/kg of bergenin , indicating that lipophilic acetylbergenin is more active against the antihepatotoxic effects of CCl4 than those of the much less lipophilic bergenin .
	manualset3
92210	1	399862	5	NULL	NULL	0	NULL	point mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , after point mutations within the promoter region occurred ( at -99 ) , new sequences appeared to which known transcription factors ( AP2 ) bind .
	manualset3
92211	2	399862	5	NULL	NULL	0	NULL	promoter region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , after point mutations within the promoter region occurred ( at -99 ) , new sequences appeared to which known transcription factors ( AP2 ) bind .
	manualset3
92212	3	399862	5	NULL	NULL	0	NULL	 -99	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , after point mutations within the promoter region occurred ( at -99 ) , new sequences appeared to which known transcription factors ( AP2 ) bind .
	manualset3
92213	4	399862	5	NULL	NULL	0	NULL	new sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , after point mutations within the promoter region occurred ( at -99 ) , new sequences appeared to which known transcription factors ( AP2 ) bind .
	manualset3
92214	5	399862	5	NULL	NULL	0	NULL	known transcription factors ( AP2 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , after point mutations within the promoter region occurred ( at -99 ) , new sequences appeared to which known transcription factors ( AP2 ) bind .
	manualset3
92215	1	399863	5	NULL	NULL	0	NULL	alcohol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , alcohol is linked to categories of disease whose relative impact on the global burden is predicted to increase .
	manualset3
92216	2	399863	5	NULL	NULL	0	NULL	categories of disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , alcohol is linked to categories of disease whose relative impact on the global burden is predicted to increase .
	manualset3
92217	3	399863	5	NULL	NULL	0	NULL	relative impact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , alcohol is linked to categories of disease whose relative impact on the global burden is predicted to increase .
	manualset3
92218	4	399863	5	NULL	NULL	0	NULL	global burden	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , alcohol is linked to categories of disease whose relative impact on the global burden is predicted to increase .
	manualset3
92219	1	399864	5	NULL	NULL	0	NULL	6 monoclonals	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , all 6 monoclonals that immunostained the enzyme in whole brain , myelin and Wolfgram protein immunoblots recognized both CNP1 ( 44 kDa ) and CNP2 ( 46 kDa ) .
	manualset3
92220	2	399864	5	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , all 6 monoclonals that immunostained the enzyme in whole brain , myelin and Wolfgram protein immunoblots recognized both CNP1 ( 44 kDa ) and CNP2 ( 46 kDa ) .
	manualset3
92221	3	399864	5	NULL	NULL	0	NULL	whole brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , all 6 monoclonals that immunostained the enzyme in whole brain , myelin and Wolfgram protein immunoblots recognized both CNP1 ( 44 kDa ) and CNP2 ( 46 kDa ) .
	manualset3
92222	4	399864	5	NULL	NULL	0	NULL	myelin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , all 6 monoclonals that immunostained the enzyme in whole brain , myelin and Wolfgram protein immunoblots recognized both CNP1 ( 44 kDa ) and CNP2 ( 46 kDa ) .
	manualset3
92223	5	399864	5	NULL	NULL	0	NULL	Wolfgram protein immunoblots	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , all 6 monoclonals that immunostained the enzyme in whole brain , myelin and Wolfgram protein immunoblots recognized both CNP1 ( 44 kDa ) and CNP2 ( 46 kDa ) .
	manualset3
92224	6	399864	5	NULL	NULL	0	NULL	CNP1 ( 44 kDa )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , all 6 monoclonals that immunostained the enzyme in whole brain , myelin and Wolfgram protein immunoblots recognized both CNP1 ( 44 kDa ) and CNP2 ( 46 kDa ) .
	manualset3
92225	7	399864	5	NULL	NULL	0	NULL	CNP2 ( 46 kDa )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , all 6 monoclonals that immunostained the enzyme in whole brain , myelin and Wolfgram protein immunoblots recognized both CNP1 ( 44 kDa ) and CNP2 ( 46 kDa ) .
	manualset3
92226	1	399865	5	NULL	NULL	0	NULL	in vitro gluing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , an in vitro gluing of the ulna segment was performed with a four-point bending test after 10 , 60 and 360 min polymerization time .
	manualset3
92227	2	399865	5	NULL	NULL	0	NULL	ulna segment	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , an in vitro gluing of the ulna segment was performed with a four-point bending test after 10 , 60 and 360 min polymerization time .
	manualset3
92228	3	399865	5	NULL	NULL	0	NULL	four-point bending test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , an in vitro gluing of the ulna segment was performed with a four-point bending test after 10 , 60 and 360 min polymerization time .
	manualset3
92229	4	399865	5	NULL	NULL	0	NULL	10 , 60 and 360 min polymerization time	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , an in vitro gluing of the ulna segment was performed with a four-point bending test after 10 , 60 and 360 min polymerization time .
	manualset3
92230	1	399866	5	NULL	NULL	0	NULL	instability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , an instability with respect to various types of periodic ordering of the two kinds of ions is found .
	manualset3
92231	2	399866	5	NULL	NULL	0	NULL	ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , an instability with respect to various types of periodic ordering of the two kinds of ions is found .
	manualset3
92232	1	399867	5	NULL	NULL	0	NULL	anterior pituitary CRF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , anterior pituitary CRF and frontal cortical 5-HT2 receptor binding was measured .
	manualset3
92233	2	399867	5	NULL	NULL	0	NULL	frontal cortical 5-HT2 receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , anterior pituitary CRF and frontal cortical 5-HT2 receptor binding was measured .
	manualset3
92234	1	399868	5	NULL	NULL	0	NULL	anthropometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , anthropometry is performed at baseline and on a yearly basis .
	manualset3
92235	2	399868	5	NULL	NULL	0	NULL	baseline	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , anthropometry is performed at baseline and on a yearly basis .
	manualset3
92821	1	399869	5	NULL	NULL	0	NULL	both modes of operation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , both modes of operation are simultaneously available , and they are mutually synchronized .
	manualset3
92236	1	399870	5	NULL	NULL	0	NULL	Staphyloccocus protease V8	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , by using Staphyloccocus protease V8 , it was possible to obtain phosphopeptides containing only serine 96 , whose phosphorylation has likewise been confirmed by radioactive labeling as well as by chemical methods .
	manualset3
92237	2	399870	5	NULL	NULL	0	NULL	phosphopeptides	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , by using Staphyloccocus protease V8 , it was possible to obtain phosphopeptides containing only serine 96 , whose phosphorylation has likewise been confirmed by radioactive labeling as well as by chemical methods .
	manualset3
92238	3	399870	5	NULL	NULL	0	NULL	serine 96	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , by using Staphyloccocus protease V8 , it was possible to obtain phosphopeptides containing only serine 96 , whose phosphorylation has likewise been confirmed by radioactive labeling as well as by chemical methods .
	manualset3
92239	4	399870	5	NULL	NULL	0	NULL	phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , by using Staphyloccocus protease V8 , it was possible to obtain phosphopeptides containing only serine 96 , whose phosphorylation has likewise been confirmed by radioactive labeling as well as by chemical methods .
	manualset3
92240	5	399870	5	NULL	NULL	0	NULL	radioactive labeling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , by using Staphyloccocus protease V8 , it was possible to obtain phosphopeptides containing only serine 96 , whose phosphorylation has likewise been confirmed by radioactive labeling as well as by chemical methods .
	manualset3
92241	6	399870	5	NULL	NULL	0	NULL	chemical methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , by using Staphyloccocus protease V8 , it was possible to obtain phosphopeptides containing only serine 96 , whose phosphorylation has likewise been confirmed by radioactive labeling as well as by chemical methods .
	manualset3
92242	1	399871	5	NULL	NULL	0	NULL	chemical and biological priming	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , chemical and biological priming provides means for triggering plant defenses in a non-transgenic manner .
	manualset3
92243	2	399871	5	NULL	NULL	0	NULL	plant defenses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , chemical and biological priming provides means for triggering plant defenses in a non-transgenic manner .
	manualset3
92244	1	399872	5	NULL	NULL	0	NULL	cholesterol feeding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , cholesterol feeding resulted in increased proportions of apo A-I and apo A-IV in the plasma VLDL fraction .
	manualset3
92245	2	399872	5	NULL	NULL	0	NULL	increased proportions	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , cholesterol feeding resulted in increased proportions of apo A-I and apo A-IV in the plasma VLDL fraction .
	manualset3
92246	3	399872	5	NULL	NULL	0	NULL	apo A-I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , cholesterol feeding resulted in increased proportions of apo A-I and apo A-IV in the plasma VLDL fraction .
	manualset3
92247	4	399872	5	NULL	NULL	0	NULL	apo A-IV	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , cholesterol feeding resulted in increased proportions of apo A-I and apo A-IV in the plasma VLDL fraction .
	manualset3
92248	5	399872	5	NULL	NULL	0	NULL	plasma VLDL fraction	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , cholesterol feeding resulted in increased proportions of apo A-I and apo A-IV in the plasma VLDL fraction .
	manualset3
92249	1	399873	5	NULL	NULL	0	NULL	comparisons	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , comparisons have been made between the results from analyses using the full range of scores on the items and those using dichotomized scores in order to determine whether the use of different rating scales for different items has an effect on the resulting item groupings .
	manualset3
92250	2	399873	5	NULL	NULL	0	NULL	result	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , comparisons have been made between the results from analyses using the full range of scores on the items and those using dichotomized scores in order to determine whether the use of different rating scales for different items has an effect on the resulting item groupings .
	manualset3
92251	3	399873	5	NULL	NULL	0	NULL	full range of scores	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , comparisons have been made between the results from analyses using the full range of scores on the items and those using dichotomized scores in order to determine whether the use of different rating scales for different items has an effect on the resulting item groupings .
	manualset3
92252	4	399873	5	NULL	NULL	0	NULL	items	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , comparisons have been made between the results from analyses using the full range of scores on the items and those using dichotomized scores in order to determine whether the use of different rating scales for different items has an effect on the resulting item groupings .
	manualset3
92253	5	399873	5	NULL	NULL	0	NULL	dichotomized scores	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , comparisons have been made between the results from analyses using the full range of scores on the items and those using dichotomized scores in order to determine whether the use of different rating scales for different items has an effect on the resulting item groupings .
	manualset3
92254	6	399873	5	NULL	NULL	0	NULL	different rating scales	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , comparisons have been made between the results from analyses using the full range of scores on the items and those using dichotomized scores in order to determine whether the use of different rating scales for different items has an effect on the resulting item groupings .
	manualset3
92255	7	399873	5	NULL	NULL	0	NULL	different items	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , comparisons have been made between the results from analyses using the full range of scores on the items and those using dichotomized scores in order to determine whether the use of different rating scales for different items has an effect on the resulting item groupings .
	manualset3
92256	8	399873	5	NULL	NULL	0	NULL	resulting item groupings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , comparisons have been made between the results from analyses using the full range of scores on the items and those using dichotomized scores in order to determine whether the use of different rating scales for different items has an effect on the resulting item groupings .
	manualset3
92257	1	399874	5	NULL	NULL	0	NULL	complicated DNA processing task	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , complicated DNA processing tasks such as the creation of libraries of DNA variants , chimeras and extensions can be accomplished with DNA processing plans consisting of multiple Y operations , which can be executed automatically under computer control .
	manualset3
92258	2	399874	5	NULL	NULL	NULL	NULL	creation of libraries of DNA variants , chimeras and extensions	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , complicated DNA processing tasks such as the creation of libraries of DNA variants , chimeras and extensions can be accomplished with DNA processing plans consisting of multiple Y operations , which can be executed automatically under computer control .
	manualset3
92259	3	399874	5	NULL	NULL	0	NULL	DNA processing plans	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , complicated DNA processing tasks such as the creation of libraries of DNA variants , chimeras and extensions can be accomplished with DNA processing plans consisting of multiple Y operations , which can be executed automatically under computer control .
	manualset3
92260	4	399874	5	NULL	NULL	0	NULL	multiple Y operations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , complicated DNA processing tasks such as the creation of libraries of DNA variants , chimeras and extensions can be accomplished with DNA processing plans consisting of multiple Y operations , which can be executed automatically under computer control .
	manualset3
92261	5	399874	5	NULL	NULL	0	NULL	computer control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , complicated DNA processing tasks such as the creation of libraries of DNA variants , chimeras and extensions can be accomplished with DNA processing plans consisting of multiple Y operations , which can be executed automatically under computer control .
	manualset3
92262	1	399875	5	NULL	NULL	0	NULL	previous findings	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , consistent with previous findings , right posterior superior frontal sulcus , and the FEF were specifically active during the delay period of the location DMS task .
	manualset3
92263	2	399875	5	NULL	NULL	0	NULL	right posterior superior frontal sulcus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , consistent with previous findings , right posterior superior frontal sulcus , and the FEF were specifically active during the delay period of the location DMS task .
	manualset3
92264	3	399875	5	NULL	NULL	0	NULL	FEF	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , consistent with previous findings , right posterior superior frontal sulcus , and the FEF were specifically active during the delay period of the location DMS task .
	manualset3
92265	4	399875	5	NULL	NULL	0	NULL	delay period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , consistent with previous findings , right posterior superior frontal sulcus , and the FEF were specifically active during the delay period of the location DMS task .
	manualset3
92266	5	399875	5	NULL	NULL	0	NULL	location DMS task	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , consistent with previous findings , right posterior superior frontal sulcus , and the FEF were specifically active during the delay period of the location DMS task .
	manualset3
92267	1	399876	5	NULL	NULL	0	NULL	Anti-inflammatory activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Anti-inflammatory activity of aqua-bis ( 2 , Y-diacetoxybenzoate ) - copper complexes ( Y = 4 , 5 or 6 ) ) .
	manualset3
92268	2	399876	5	NULL	NULL	0	NULL	aqua-bis ( 2 , Y-diacetoxybenzoate ) - copper complexes ( Y = 4 , 5 or 6 )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Anti-inflammatory activity of aqua-bis ( 2 , Y-diacetoxybenzoate ) - copper complexes ( Y = 4 , 5 or 6 ) ) .
	manualset3
92269	1	399877	5	NULL	NULL	0	NULL	human anti-Rh ( D ) immunoglobulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Use of human anti-Rh ( D ) immunoglobulin ) .
	manualset3
92270	1	399878	5	NULL	NULL	0	NULL	cytotoxic effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , cytotoxic effects were also studied in normal human fibroblasts that represent normal tissue and the results are compared to the tumor cell lines .
	manualset3
92271	2	399878	5	NULL	NULL	0	NULL	normal human fibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , cytotoxic effects were also studied in normal human fibroblasts that represent normal tissue and the results are compared to the tumor cell lines .
	manualset3
92272	3	399878	5	NULL	NULL	0	NULL	normal tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , cytotoxic effects were also studied in normal human fibroblasts that represent normal tissue and the results are compared to the tumor cell lines .
	manualset3
92273	4	399878	5	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , cytotoxic effects were also studied in normal human fibroblasts that represent normal tissue and the results are compared to the tumor cell lines .
	manualset3
92274	5	399878	5	NULL	NULL	0	NULL	tumor cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , cytotoxic effects were also studied in normal human fibroblasts that represent normal tissue and the results are compared to the tumor cell lines .
	manualset3
92275	1	399879	5	NULL	NULL	0	NULL	depot preparations	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , depot preparations of vitamins D and A and possibly iron should be provided for curative and prophylactic purposes .
	manualset3
92276	2	399879	5	NULL	NULL	NULL	NULL	vitamin D	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , depot preparations of vitamins D and A and possibly iron should be provided for curative and prophylactic purposes .
	manualset3
92277	3	399879	5	NULL	NULL	0	NULL	iron	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , depot preparations of vitamins D and A and possibly iron should be provided for curative and prophylactic purposes .
	manualset3
92278	4	399879	5	NULL	NULL	0	NULL	curative and prophylactic purposes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , depot preparations of vitamins D and A and possibly iron should be provided for curative and prophylactic purposes .
	manualset3
93340	5	399879	5	NULL	NULL	0	NULL	vitamin A	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , depot preparations of vitamins D and A and possibly iron should be provided for curative and prophylactic purposes .
	manualset3
92279	1	399880	5	NULL	NULL	NULL	NULL	derivatization of teh probe	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , derivatization of the probe enabled the labeling of intracellular proteins and the modification of various functional molecules .
	manualset3
92280	2	399880	5	NULL	NULL	0	NULL	intracellular proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , derivatization of the probe enabled the labeling of intracellular proteins and the modification of various functional molecules .
	manualset3
92281	3	399880	5	NULL	NULL	0	NULL	functional molecules	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , derivatization of the probe enabled the labeling of intracellular proteins and the modification of various functional molecules .
	manualset3
92282	1	399881	5	NULL	NULL	0	NULL	detection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , detection of cell surface markers such as CD 33 , CD 34 , CD 68 , CD 99 , and HLA-DR may be useful .
	manualset3
92283	2	399881	5	NULL	NULL	NULL	NULL	cell surface markers	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , detection of cell surface markers such as CD 33 , CD 34 , CD 68 , CD 99 , and HLA-DR may be useful .
	manualset3
92284	3	399881	5	NULL	NULL	0	NULL	CD 33	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , detection of cell surface markers such as CD 33 , CD 34 , CD 68 , CD 99 , and HLA-DR may be useful .
	manualset3
92285	4	399881	5	NULL	NULL	0	NULL	CD 34	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , detection of cell surface markers such as CD 33 , CD 34 , CD 68 , CD 99 , and HLA-DR may be useful .
	manualset3
92286	5	399881	5	NULL	NULL	0	NULL	CD 68	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , detection of cell surface markers such as CD 33 , CD 34 , CD 68 , CD 99 , and HLA-DR may be useful .
	manualset3
92287	6	399881	5	NULL	NULL	0	NULL	CD 99	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , detection of cell surface markers such as CD 33 , CD 34 , CD 68 , CD 99 , and HLA-DR may be useful .
	manualset3
92288	7	399881	5	NULL	NULL	0	NULL	HLA-DR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , detection of cell surface markers such as CD 33 , CD 34 , CD 68 , CD 99 , and HLA-DR may be useful .
	manualset3
92289	1	399882	5	NULL	NULL	0	NULL	developmental delay	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , developmental delay in some 45 , X males may be related to specific deletion of telomeric autosome regions , but involvement of gene ( s ) on the Y chromosome may play a role as well .
	manualset3
92290	2	399882	5	NULL	NULL	0	NULL	45 , X males	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , developmental delay in some 45 , X males may be related to specific deletion of telomeric autosome regions , but involvement of gene ( s ) on the Y chromosome may play a role as well .
	manualset3
92291	3	399882	5	NULL	NULL	0	NULL	specific deletion of telomeric autosome regions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , developmental delay in some 45 , X males may be related to specific deletion of telomeric autosome regions , but involvement of gene ( s ) on the Y chromosome may play a role as well .
	manualset3
92292	4	399882	5	NULL	NULL	0	NULL	involvement of gene ( s )	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , developmental delay in some 45 , X males may be related to specific deletion of telomeric autosome regions , but involvement of gene ( s ) on the Y chromosome may play a role as well .
	manualset3
92293	5	399882	5	NULL	NULL	0	NULL	Y chromosome	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , developmental delay in some 45 , X males may be related to specific deletion of telomeric autosome regions , but involvement of gene ( s ) on the Y chromosome may play a role as well .
	manualset3
92294	6	399882	5	NULL	NULL	NULL	NULL	role	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , developmental delay in some 45 , X males may be related to specific deletion of telomeric autosome regions , but involvement of gene ( s ) on the Y chromosome may play a role as well .
	manualset3
92295	1	399883	5	NULL	NULL	0	NULL	electron paramagnetic resonance studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , electron paramagnetic resonance studies showed that in systems containing the reductase plus NADH , levels of chromanoxyl radicals were dramatically reduced .
	manualset3
92296	2	399883	5	NULL	NULL	NULL	NULL	systems containing the reductase plus NADH	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , electron paramagnetic resonance studies showed that in systems containing the reductase plus NADH , levels of chromanoxyl radicals were dramatically reduced .
	manualset3
92298	3	399883	5	NULL	NULL	0	NULL	levels of chromanoxyl radicals	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , electron paramagnetic resonance studies showed that in systems containing the reductase plus NADH , levels of chromanoxyl radicals were dramatically reduced .
	manualset3
92299	1	399884	5	NULL	NULL	0	NULL	electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , electrophoresis of oviduct nuclear RNA on agarose gels containing methylmercury hydroxide reveals multiple species of RNA that are from 1.3 to over 4 times larger than ovalbumin mRNA and hybridize to both structural and intervening sequences of the ovalbumin gene .
	manualset3
92300	2	399884	5	NULL	NULL	0	NULL	oviduct nuclear RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , electrophoresis of oviduct nuclear RNA on agarose gels containing methylmercury hydroxide reveals multiple species of RNA that are from 1.3 to over 4 times larger than ovalbumin mRNA and hybridize to both structural and intervening sequences of the ovalbumin gene .
	manualset3
92301	3	399884	5	NULL	NULL	0	NULL	agarose gels	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , electrophoresis of oviduct nuclear RNA on agarose gels containing methylmercury hydroxide reveals multiple species of RNA that are from 1.3 to over 4 times larger than ovalbumin mRNA and hybridize to both structural and intervening sequences of the ovalbumin gene .
	manualset3
92302	4	399884	5	NULL	NULL	0	NULL	methylmercury hydroxide	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , electrophoresis of oviduct nuclear RNA on agarose gels containing methylmercury hydroxide reveals multiple species of RNA that are from 1.3 to over 4 times larger than ovalbumin mRNA and hybridize to both structural and intervening sequences of the ovalbumin gene .
	manualset3
92303	5	399884	5	NULL	NULL	0	NULL	multiple species of RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , electrophoresis of oviduct nuclear RNA on agarose gels containing methylmercury hydroxide reveals multiple species of RNA that are from 1.3 to over 4 times larger than ovalbumin mRNA and hybridize to both structural and intervening sequences of the ovalbumin gene .
	manualset3
92304	6	399884	5	NULL	NULL	0	NULL	1.3 to over 4 times larger	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , electrophoresis of oviduct nuclear RNA on agarose gels containing methylmercury hydroxide reveals multiple species of RNA that are from 1.3 to over 4 times larger than ovalbumin mRNA and hybridize to both structural and intervening sequences of the ovalbumin gene .
	manualset3
92305	7	399884	5	NULL	NULL	0	NULL	ovalbumin mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , electrophoresis of oviduct nuclear RNA on agarose gels containing methylmercury hydroxide reveals multiple species of RNA that are from 1.3 to over 4 times larger than ovalbumin mRNA and hybridize to both structural and intervening sequences of the ovalbumin gene .
	manualset3
92306	8	399884	5	NULL	NULL	0	NULL	structural and intervening sequences of the ovalbumin gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , electrophoresis of oviduct nuclear RNA on agarose gels containing methylmercury hydroxide reveals multiple species of RNA that are from 1.3 to over 4 times larger than ovalbumin mRNA and hybridize to both structural and intervening sequences of the ovalbumin gene .
	manualset3
92307	1	399885	5	NULL	NULL	0	NULL	equal rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , equal rates of hypotension ( 18.5 % vs 17.2 % ) were noted between the groups .
	manualset3
92308	2	399885	5	NULL	NULL	0	NULL	hypotension	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , equal rates of hypotension ( 18.5 % vs 17.2 % ) were noted between the groups .
	manualset3
92309	3	399885	5	NULL	NULL	0	NULL	18.5 % vs 17.2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , equal rates of hypotension ( 18.5 % vs 17.2 % ) were noted between the groups .
	manualset3
92310	4	399885	5	NULL	NULL	0	NULL	groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , equal rates of hypotension ( 18.5 % vs 17.2 % ) were noted between the groups .
	manualset3
92311	1	399886	5	NULL	NULL	0	NULL	evidence	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , evidence has been obtained concerning the structure of Dictyostelium rDNA which agrees with the finding ( Taylor et al. ( 1977 ) ICN-UCLA Symp .
	manualset3
92312	2	399886	5	NULL	NULL	0	NULL	structure of Dictyostelium rDNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , evidence has been obtained concerning the structure of Dictyostelium rDNA which agrees with the finding ( Taylor et al. ( 1977 ) ICN-UCLA Symp .
	manualset3
92313	3	399886	5	NULL	NULL	NULL	NULL	Taylor et al. ( 1977 ) ICN-UCLA Symp	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , evidence has been obtained concerning the structure of Dictyostelium rDNA which agrees with the finding ( Taylor et al. ( 1977 ) ICN-UCLA Symp .
	manualset3
92315	1	399887	5	NULL	NULL	0	NULL	indirect hemagglutination test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Use of the indirect hemagglutination test in the study of ornithosis .
	manualset3
92316	2	399887	5	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Use of the indirect hemagglutination test in the study of ornithosis .
	manualset3
92317	3	399887	5	NULL	NULL	0	NULL	ornithosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Use of the indirect hemagglutination test in the study of ornithosis .
	manualset3
92318	1	399888	5	NULL	NULL	0	NULL	family practitioners	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , family practitioners see a different kind of patient than speciality physicians and may not have immediate access to diagnostic investigations .
	manualset3
92319	2	399888	5	NULL	NULL	0	NULL	different kind of patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , family practitioners see a different kind of patient than speciality physicians and may not have immediate access to diagnostic investigations .
	manualset3
92320	3	399888	5	NULL	NULL	0	NULL	speciality physicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , family practitioners see a different kind of patient than speciality physicians and may not have immediate access to diagnostic investigations .
	manualset3
92321	4	399888	5	NULL	NULL	0	NULL	immediate access	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , family practitioners see a different kind of patient than speciality physicians and may not have immediate access to diagnostic investigations .
	manualset3
92322	5	399888	5	NULL	NULL	NULL	NULL	diagnostic investigations	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , family practitioners see a different kind of patient than speciality physicians and may not have immediate access to diagnostic investigations .
	manualset3
92323	1	399889	5	NULL	NULL	0	NULL	older group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , for the older group , but not for the younger one , intentional instructions impaired implicit pattern learning .
	manualset3
92324	2	399889	5	NULL	NULL	NULL	NULL	younger one	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , for the older group , but not for the younger one , intentional instructions impaired implicit pattern learning .
	manualset3
92325	3	399889	5	NULL	NULL	0	NULL	intentional instructions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , for the older group , but not for the younger one , intentional instructions impaired implicit pattern learning .
	manualset3
92326	4	399889	5	NULL	NULL	0	NULL	 implicit pattern learning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , for the older group , but not for the younger one , intentional instructions impaired implicit pattern learning .
	manualset3
92327	1	399890	5	NULL	NULL	0	NULL	generic medications	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , generic medications such as statins might be able to moderate the aberrant innate immune response that characterizes human cases of H5N1 influenza .
	manualset3
92328	2	399890	5	NULL	NULL	0	NULL	statins	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , generic medications such as statins might be able to moderate the aberrant innate immune response that characterizes human cases of H5N1 influenza .
	manualset3
92329	3	399890	5	NULL	NULL	0	NULL	aberrant innate immune response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , generic medications such as statins might be able to moderate the aberrant innate immune response that characterizes human cases of H5N1 influenza .
	manualset3
92330	4	399890	5	NULL	NULL	NULL	NULL	human cases of H5N1 influenza	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , generic medications such as statins might be able to moderate the aberrant innate immune response that characterizes human cases of H5N1 influenza .
	manualset3
92332	1	399891	5	NULL	NULL	0	NULL	 heterologous and endothelium-dependent desensitization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , heterologous and endothelium-dependent desensitization induced by noradrenaline and angiotensin II on the contractile response to each other was found .
	manualset3
92333	2	399891	5	NULL	NULL	0	NULL	noradrenaline	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , heterologous and endothelium-dependent desensitization induced by noradrenaline and angiotensin II on the contractile response to each other was found .
	manualset3
92334	3	399891	5	NULL	NULL	0	NULL	angiotensin II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , heterologous and endothelium-dependent desensitization induced by noradrenaline and angiotensin II on the contractile response to each other was found .
	manualset3
92335	4	399891	5	NULL	NULL	0	NULL	contractile response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , heterologous and endothelium-dependent desensitization induced by noradrenaline and angiotensin II on the contractile response to each other was found .
	manualset3
92336	1	399892	5	NULL	NULL	0	NULL	high dose ( 2 mg ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , high dose ( 2 mg ) of ibutilide was more effective than sotalol ( 1.5 mg/kg ) in conversion of Aflut to SR ( 70 versus 19 % ) .
	manualset3
92337	2	399892	5	NULL	NULL	0	NULL	ibutilide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , high dose ( 2 mg ) of ibutilide was more effective than sotalol ( 1.5 mg/kg ) in conversion of Aflut to SR ( 70 versus 19 % ) .
	manualset3
92338	3	399892	5	NULL	NULL	0	NULL	sotalol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , high dose ( 2 mg ) of ibutilide was more effective than sotalol ( 1.5 mg/kg ) in conversion of Aflut to SR ( 70 versus 19 % ) .
	manualset3
92339	4	399892	5	NULL	NULL	0	NULL	1.5 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , high dose ( 2 mg ) of ibutilide was more effective than sotalol ( 1.5 mg/kg ) in conversion of Aflut to SR ( 70 versus 19 % ) .
	manualset3
92340	5	399892	5	NULL	NULL	0	NULL	conversion of Aflut to SR	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , high dose ( 2 mg ) of ibutilide was more effective than sotalol ( 1.5 mg/kg ) in conversion of Aflut to SR ( 70 versus 19 % ) .
	manualset3
92341	6	399892	5	NULL	NULL	0	NULL	70 versus 19 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , high dose ( 2 mg ) of ibutilide was more effective than sotalol ( 1.5 mg/kg ) in conversion of Aflut to SR ( 70 versus 19 % ) .
	manualset3
92342	1	399893	5	NULL	NULL	0	NULL	immunoassays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , immunoassays may be more sensitive than GC-MS for detecting LSD use as current confirmation assays are targeted towards detection of the parent drug only .
	manualset3
92343	2	399893	5	NULL	NULL	0	NULL	GC-MS	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , immunoassays may be more sensitive than GC-MS for detecting LSD use as current confirmation assays are targeted towards detection of the parent drug only .
	manualset3
92344	3	399893	5	NULL	NULL	0	NULL	LSD	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , immunoassays may be more sensitive than GC-MS for detecting LSD use as current confirmation assays are targeted towards detection of the parent drug only .
	manualset3
92345	4	399893	5	NULL	NULL	0	NULL	current confirmation assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , immunoassays may be more sensitive than GC-MS for detecting LSD use as current confirmation assays are targeted towards detection of the parent drug only .
	manualset3
92346	5	399893	5	NULL	NULL	0	NULL	detection of the parent drug	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , immunoassays may be more sensitive than GC-MS for detecting LSD use as current confirmation assays are targeted towards detection of the parent drug only .
	manualset3
92347	5	399893	5	NULL	NULL	0	NULL	detection of the parent drug	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , immunoassays may be more sensitive than GC-MS for detecting LSD use as current confirmation assays are targeted towards detection of the parent drug only .
	manualset3
92348	1	399894	5	NULL	NULL	NULL	NULL	intralitter variability	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , in order to evaluate the significance of intralitter variability in fetal SCE responses , SCE in combined ( `` pooled '' ) fetal liver tissue preparations were measured and compared with average individual responses .
	manualset3
92349	2	399894	5	NULL	NULL	0	NULL	fetal SCE responses	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , in order to evaluate the significance of intralitter variability in fetal SCE responses , SCE in combined ( `` pooled '' ) fetal liver tissue preparations were measured and compared with average individual responses .
	manualset3
92350	3	399894	5	NULL	NULL	0	NULL	SCE	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , in order to evaluate the significance of intralitter variability in fetal SCE responses , SCE in combined ( `` pooled '' ) fetal liver tissue preparations were measured and compared with average individual responses .
	manualset3
92351	4	399894	5	NULL	NULL	0	NULL	combined ( `` pooled '' ) fetal liver tissue preparations	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , in order to evaluate the significance of intralitter variability in fetal SCE responses , SCE in combined ( `` pooled '' ) fetal liver tissue preparations were measured and compared with average individual responses .
	manualset3
92352	5	399894	5	NULL	NULL	0	NULL	average individual responses	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , in order to evaluate the significance of intralitter variability in fetal SCE responses , SCE in combined ( `` pooled '' ) fetal liver tissue preparations were measured and compared with average individual responses .
	manualset3
92353	1	399895	5	NULL	NULL	0	NULL	case	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , in the case of the deuterium exchanged proteins a 2H1H quadrupole dip appears .
	manualset3
92354	2	399895	5	NULL	NULL	0	NULL	deuterium exchanged proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , in the case of the deuterium exchanged proteins a 2H1H quadrupole dip appears .
	manualset3
92355	3	399895	5	NULL	NULL	0	NULL	2H1H quadrupole dip	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , in the case of the deuterium exchanged proteins a 2H1H quadrupole dip appears .
	manualset3
92356	1	399896	5	NULL	NULL	0	NULL	conformational features	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , insight into conformational features of azapeptides in general in comparison with the corresponding purely peptidic compounds is given .
	manualset3
92357	2	399896	5	NULL	NULL	0	NULL	azapeptides	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , insight into conformational features of azapeptides in general in comparison with the corresponding purely peptidic compounds is given .
	manualset3
92358	3	399896	5	NULL	NULL	0	NULL	 corresponding purely peptidic compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , insight into conformational features of azapeptides in general in comparison with the corresponding purely peptidic compounds is given .
	manualset3
92359	1	399897	5	NULL	NULL	0	NULL	changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , it is difficult to make changes in underlying data storage without affecting the visualisation interface .
	manualset3
92360	2	399897	5	NULL	NULL	0	NULL	underlying data storage	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , it is difficult to make changes in underlying data storage without affecting the visualisation interface .
	manualset3
92361	3	399897	5	NULL	NULL	0	NULL	visualisation interface	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , it is difficult to make changes in underlying data storage without affecting the visualisation interface .
	manualset3
92362	1	399898	5	NULL	NULL	0	NULL	signet ring	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , it is suggested that both signet ring and rhabdoid are not appropriate because they do not reflect histogenesis and are not necessarily reflective of tumor biology .
	manualset3
92363	2	399898	5	NULL	NULL	0	NULL	rhabdoid	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , it is suggested that both signet ring and rhabdoid are not appropriate because they do not reflect histogenesis and are not necessarily reflective of tumor biology .
	manualset3
92364	3	399898	5	NULL	NULL	0	NULL	histogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , it is suggested that both signet ring and rhabdoid are not appropriate because they do not reflect histogenesis and are not necessarily reflective of tumor biology .
	manualset3
92365	4	399898	5	NULL	NULL	0	NULL	tumor biology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , it is suggested that both signet ring and rhabdoid are not appropriate because they do not reflect histogenesis and are not necessarily reflective of tumor biology .
	manualset3
92366	1	399899	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , it was demonstrated that patients suffering from aphasia as well as temporal and `` frontal lobe '' damage perform at a level higher than suspected malingerers .
	manualset3
92367	2	399899	5	NULL	NULL	0	NULL	aphasia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , it was demonstrated that patients suffering from aphasia as well as temporal and `` frontal lobe '' damage perform at a level higher than suspected malingerers .
	manualset3
92368	3	399899	5	NULL	NULL	0	NULL	temporal and `` frontal lobe '' damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , it was demonstrated that patients suffering from aphasia as well as temporal and `` frontal lobe '' damage perform at a level higher than suspected malingerers .
	manualset3
92369	4	399899	5	NULL	NULL	0	NULL	level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , it was demonstrated that patients suffering from aphasia as well as temporal and `` frontal lobe '' damage perform at a level higher than suspected malingerers .
	manualset3
92371	5	399899	5	NULL	NULL	0	NULL	malingerers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , it was demonstrated that patients suffering from aphasia as well as temporal and `` frontal lobe '' damage perform at a level higher than suspected malingerers .
	manualset3
92372	1	399900	5	NULL	NULL	0	NULL	antineoplastic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , its antineoplastic activity toward colon-rectum cancers has been documented both in vivo and in vitro .
	manualset3
92373	2	399900	5	NULL	NULL	0	NULL	colon-rectum cancers	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , its antineoplastic activity toward colon-rectum cancers has been documented both in vivo and in vitro .
	manualset3
92374	1	399901	5	NULL	NULL	0	NULL	ligand-activated ER	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , ligand-activated ER can interact with other factors to alter the physiology and growth of cells .
	manualset3
92375	2	399901	5	NULL	NULL	0	NULL	other factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , ligand-activated ER can interact with other factors to alter the physiology and growth of cells .
	manualset3
92376	3	399901	5	NULL	NULL	0	NULL	physiology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , ligand-activated ER can interact with other factors to alter the physiology and growth of cells .
	manualset3
92377	4	399901	5	NULL	NULL	0	NULL	growth of cells	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , ligand-activated ER can interact with other factors to alter the physiology and growth of cells .
	manualset3
92378	1	399902	5	NULL	NULL	NULL	NULL	new and exciting roles	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , many new and exciting roles for ET-1 were presented , suggesting that ET-1 antagonism may have a broader therapeutic potential than previously imagined .
	manualset3
92379	2	399902	5	NULL	NULL	0	NULL	ET-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , many new and exciting roles for ET-1 were presented , suggesting that ET-1 antagonism may have a broader therapeutic potential than previously imagined .
	manualset3
92380	3	399902	5	NULL	NULL	0	NULL	ET-1 antagonism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , many new and exciting roles for ET-1 were presented , suggesting that ET-1 antagonism may have a broader therapeutic potential than previously imagined .
	manualset3
92381	4	399902	5	NULL	NULL	0	NULL	broader therapeutic potential	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , many new and exciting roles for ET-1 were presented , suggesting that ET-1 antagonism may have a broader therapeutic potential than previously imagined .
	manualset3
92382	1	399903	5	NULL	NULL	0	NULL	measures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , measures of maternal orientation ( PPQ ) , personality ( NEO-FFI ) , coping styles ( UCL ) , adult attachment ( RQ ) , and parental bonding ( PBI ) were completed antenatally .
	manualset3
92383	2	399903	5	NULL	NULL	0	NULL	maternal orientation ( PPQ )	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , measures of maternal orientation ( PPQ ) , personality ( NEO-FFI ) , coping styles ( UCL ) , adult attachment ( RQ ) , and parental bonding ( PBI ) were completed antenatally .
	manualset3
92384	3	399903	5	NULL	NULL	0	NULL	personality ( NEO-FFI )	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , measures of maternal orientation ( PPQ ) , personality ( NEO-FFI ) , coping styles ( UCL ) , adult attachment ( RQ ) , and parental bonding ( PBI ) were completed antenatally .
	manualset3
92385	4	399903	5	NULL	NULL	0	NULL	coping styles ( UCL )	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , measures of maternal orientation ( PPQ ) , personality ( NEO-FFI ) , coping styles ( UCL ) , adult attachment ( RQ ) , and parental bonding ( PBI ) were completed antenatally .
	manualset3
92386	5	399903	5	NULL	NULL	0	NULL	adult attachment ( RQ )	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , measures of maternal orientation ( PPQ ) , personality ( NEO-FFI ) , coping styles ( UCL ) , adult attachment ( RQ ) , and parental bonding ( PBI ) were completed antenatally .
	manualset3
92387	6	399903	5	NULL	NULL	0	NULL	parental bonding ( PBI )	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , measures of maternal orientation ( PPQ ) , personality ( NEO-FFI ) , coping styles ( UCL ) , adult attachment ( RQ ) , and parental bonding ( PBI ) were completed antenatally .
	manualset3
92388	1	399904	5	NULL	NULL	0	NULL	morphology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , morphology and mechanical properties of the 3D constructs were examined .
	manualset3
92389	2	399904	5	NULL	NULL	0	NULL	mechanical properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , morphology and mechanical properties of the 3D constructs were examined .
	manualset3
92390	3	399904	5	NULL	NULL	0	NULL	3D constructs	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , morphology and mechanical properties of the 3D constructs were examined .
	manualset3
92391	1	399905	5	NULL	NULL	0	NULL	three-dimensional reconstruction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Use of three-dimensional reconstruction of the biliary tree in spiral computed tomography without using hepatotropic contrast media ) .
	manualset3
92392	2	399905	5	NULL	NULL	0	NULL	biliary tree	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Use of three-dimensional reconstruction of the biliary tree in spiral computed tomography without using hepatotropic contrast media ) .
	manualset3
92393	3	399905	5	NULL	NULL	0	NULL	spiral computed tomography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Use of three-dimensional reconstruction of the biliary tree in spiral computed tomography without using hepatotropic contrast media ) .
	manualset3
92394	4	399905	5	NULL	NULL	0	NULL	hepatotropic contrast media	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	( Use of three-dimensional reconstruction of the biliary tree in spiral computed tomography without using hepatotropic contrast media ) .
	manualset3
92395	1	399906	5	NULL	NULL	0	NULL	log K ( f ) values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , no significant differences in the log K ( f ) values of all analytes except for PCB 206 were found between the sample sizes of 130 mL and 2 L for both the 7 - and 100-microm coatings .
	manualset3
92396	2	399906	5	NULL	NULL	0	NULL	analytes	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , no significant differences in the log K ( f ) values of all analytes except for PCB 206 were found between the sample sizes of 130 mL and 2 L for both the 7 - and 100-microm coatings .
	manualset3
92398	3	399906	5	NULL	NULL	0	NULL	PCB 206	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , no significant differences in the log K ( f ) values of all analytes except for PCB 206 were found between the sample sizes of 130 mL and 2 L for both the 7 - and 100-microm coatings .
	manualset3
92399	4	399906	5	NULL	NULL	0	NULL	sample sizes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , no significant differences in the log K ( f ) values of all analytes except for PCB 206 were found between the sample sizes of 130 mL and 2 L for both the 7 - and 100-microm coatings .
	manualset3
92400	5	399906	5	NULL	NULL	0	NULL	130 mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , no significant differences in the log K ( f ) values of all analytes except for PCB 206 were found between the sample sizes of 130 mL and 2 L for both the 7 - and 100-microm coatings .
	manualset3
92401	6	399906	5	NULL	NULL	0	NULL	2 L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , no significant differences in the log K ( f ) values of all analytes except for PCB 206 were found between the sample sizes of 130 mL and 2 L for both the 7 - and 100-microm coatings .
	manualset3
92402	7	399906	5	NULL	NULL	0	NULL	7 - and 100-microm coatings	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , no significant differences in the log K ( f ) values of all analytes except for PCB 206 were found between the sample sizes of 130 mL and 2 L for both the 7 - and 100-microm coatings .
	manualset3
92403	1	399907	5	NULL	NULL	0	NULL	minimal sample volume	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , only a minimal sample volume is required , enabling studies even in very small subjects , such as preterm infants .
	manualset3
92404	2	399907	5	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , only a minimal sample volume is required , enabling studies even in very small subjects , such as preterm infants .
	manualset3
92405	3	399907	5	NULL	NULL	0	NULL	very small subjects , such as preterm infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , only a minimal sample volume is required , enabling studies even in very small subjects , such as preterm infants .
	manualset3
92407	1	399908	5	NULL	NULL	0	NULL	partial complexes	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , partial complexes were generated by immunoprecipitation with antibodies that cause selective dissociation of T-cell antigen receptor chains .
	manualset3
92408	2	399908	5	NULL	NULL	0	NULL	immunoprecipitation with antibodies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , partial complexes were generated by immunoprecipitation with antibodies that cause selective dissociation of T-cell antigen receptor chains .
	manualset3
92409	3	399908	5	NULL	NULL	0	NULL	selective dissociation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , partial complexes were generated by immunoprecipitation with antibodies that cause selective dissociation of T-cell antigen receptor chains .
	manualset3
92413	4	399908	5	NULL	NULL	0	NULL	T-cell antigen receptor chains	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , partial complexes were generated by immunoprecipitation with antibodies that cause selective dissociation of T-cell antigen receptor chains .
	manualset3
92415	1	399909	5	NULL	NULL	0	NULL	persons with mild disease	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , persons with mild disease should be promptly informed of their diagnosis in order to obtain their wishes regarding life prolonging measures and extended care options .
	manualset3
92416	2	399909	5	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , persons with mild disease should be promptly informed of their diagnosis in order to obtain their wishes regarding life prolonging measures and extended care options .
	manualset3
92417	3	399909	5	NULL	NULL	0	NULL	wishes	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , persons with mild disease should be promptly informed of their diagnosis in order to obtain their wishes regarding life prolonging measures and extended care options .
	manualset3
92418	4	399909	5	NULL	NULL	0	NULL	life prolonging measures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , persons with mild disease should be promptly informed of their diagnosis in order to obtain their wishes regarding life prolonging measures and extended care options .
	manualset3
92420	5	399909	5	NULL	NULL	0	NULL	extended care options	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , persons with mild disease should be promptly informed of their diagnosis in order to obtain their wishes regarding life prolonging measures and extended care options .
	manualset3
92426	1	399910	5	NULL	NULL	NULL	NULL	 post-HD PBMC	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , post-HD PBMC produced significantly more TNF alpha than pre-HD PBMC suggesting that the HD procedure itself may activate cytokine production .
	manualset3
92429	2	399910	5	NULL	NULL	NULL	NULL	TNF alpha	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , post-HD PBMC produced significantly more TNF alpha than pre-HD PBMC suggesting that the HD procedure itself may activate cytokine production .
	manualset3
92431	3	399910	5	NULL	NULL	0	NULL	pre-HD PBMC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , post-HD PBMC produced significantly more TNF alpha than pre-HD PBMC suggesting that the HD procedure itself may activate cytokine production .
	manualset3
92432	4	399910	5	NULL	NULL	0	NULL	HD procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , post-HD PBMC produced significantly more TNF alpha than pre-HD PBMC suggesting that the HD procedure itself may activate cytokine production .
	manualset3
92433	5	399910	5	NULL	NULL	0	NULL	cytokine production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , post-HD PBMC produced significantly more TNF alpha than pre-HD PBMC suggesting that the HD procedure itself may activate cytokine production .
	manualset3
92434	1	399911	5	NULL	NULL	0	NULL	 prolonged incubation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , prolonged incubation of PDE6 with vardenafil or sildenafil ( but not 3-isobutyl-1-methylxanthine and zaprinast ) induced a distinct conformational change in the catalytic domain without affecting the binding properties of the GAF domains .
	manualset3
92435	2	399911	5	NULL	NULL	0	NULL	PDE6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , prolonged incubation of PDE6 with vardenafil or sildenafil ( but not 3-isobutyl-1-methylxanthine and zaprinast ) induced a distinct conformational change in the catalytic domain without affecting the binding properties of the GAF domains .
	manualset3
92436	3	399911	5	NULL	NULL	0	NULL	vardenafil	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , prolonged incubation of PDE6 with vardenafil or sildenafil ( but not 3-isobutyl-1-methylxanthine and zaprinast ) induced a distinct conformational change in the catalytic domain without affecting the binding properties of the GAF domains .
	manualset3
92437	4	399911	5	NULL	NULL	0	NULL	sildenafil	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , prolonged incubation of PDE6 with vardenafil or sildenafil ( but not 3-isobutyl-1-methylxanthine and zaprinast ) induced a distinct conformational change in the catalytic domain without affecting the binding properties of the GAF domains .
	manualset3
92439	5	399911	5	NULL	NULL	NULL	NULL	3-isobutyl-1-methylxanthine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , prolonged incubation of PDE6 with vardenafil or sildenafil ( but not 3-isobutyl-1-methylxanthine and zaprinast ) induced a distinct conformational change in the catalytic domain without affecting the binding properties of the GAF domains .
	manualset3
92440	6	399911	5	NULL	NULL	0	NULL	zaprinast	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , prolonged incubation of PDE6 with vardenafil or sildenafil ( but not 3-isobutyl-1-methylxanthine and zaprinast ) induced a distinct conformational change in the catalytic domain without affecting the binding properties of the GAF domains .
	manualset3
92441	7	399911	5	NULL	NULL	0	NULL	distinct conformational change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , prolonged incubation of PDE6 with vardenafil or sildenafil ( but not 3-isobutyl-1-methylxanthine and zaprinast ) induced a distinct conformational change in the catalytic domain without affecting the binding properties of the GAF domains .
	manualset3
92442	8	399911	5	NULL	NULL	0	NULL	catalytic domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , prolonged incubation of PDE6 with vardenafil or sildenafil ( but not 3-isobutyl-1-methylxanthine and zaprinast ) induced a distinct conformational change in the catalytic domain without affecting the binding properties of the GAF domains .
	manualset3
92443	9	399911	5	NULL	NULL	0	NULL	binding properties 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , prolonged incubation of PDE6 with vardenafil or sildenafil ( but not 3-isobutyl-1-methylxanthine and zaprinast ) induced a distinct conformational change in the catalytic domain without affecting the binding properties of the GAF domains .
	manualset3
92444	10	399911	5	NULL	NULL	0	NULL	GAF domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , prolonged incubation of PDE6 with vardenafil or sildenafil ( but not 3-isobutyl-1-methylxanthine and zaprinast ) induced a distinct conformational change in the catalytic domain without affecting the binding properties of the GAF domains .
	manualset3
92445	1	399912	5	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Use of water in Leskovac ) .
	manualset3
92446	2	399912	5	NULL	NULL	0	NULL	Leskovac	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Use of water in Leskovac ) .
	manualset3
92447	1	399913	5	NULL	NULL	0	NULL	protozoa numbers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , protozoa numbers in fermenters were 121 and 226 times lower than those in the sheep rumen for HF and HC diets , respectively .
	manualset3
92448	2	399913	5	NULL	NULL	0	NULL	fermenters	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , protozoa numbers in fermenters were 121 and 226 times lower than those in the sheep rumen for HF and HC diets , respectively .
	manualset3
92449	3	399913	5	NULL	NULL	NULL	NULL	121 and 226 times	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , protozoa numbers in fermenters were 121 and 226 times lower than those in the sheep rumen for HF and HC diets , respectively .
	manualset3
92451	4	399913	5	NULL	NULL	NULL	NULL	sheep rumen	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , protozoa numbers in fermenters were 121 and 226 times lower than those in the sheep rumen for HF and HC diets , respectively .
	manualset3
92452	5	399913	5	NULL	NULL	NULL	NULL	HF diet	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , protozoa numbers in fermenters were 121 and 226 times lower than those in the sheep rumen for HF and HC diets , respectively .
	manualset3
93341	6	399913	5	NULL	NULL	0	NULL	HC diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , protozoa numbers in fermenters were 121 and 226 times lower than those in the sheep rumen for HF and HC diets , respectively .
	manualset3
92453	1	399914	5	NULL	NULL	0	NULL	recent developments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , recent developments in the area of evaluation and management services over the last few months are of significance to interventional pain physicians .
	manualset3
92454	2	399914	5	NULL	NULL	0	NULL	area	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , recent developments in the area of evaluation and management services over the last few months are of significance to interventional pain physicians .
	manualset3
92455	3	399914	5	NULL	NULL	0	NULL	evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , recent developments in the area of evaluation and management services over the last few months are of significance to interventional pain physicians .
	manualset3
92456	4	399914	5	NULL	NULL	0	NULL	management services	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , recent developments in the area of evaluation and management services over the last few months are of significance to interventional pain physicians .
	manualset3
92457	5	399914	5	NULL	NULL	0	NULL	over the last few months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , recent developments in the area of evaluation and management services over the last few months are of significance to interventional pain physicians .
	manualset3
92458	6	399914	5	NULL	NULL	0	NULL	interventional pain physicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , recent developments in the area of evaluation and management services over the last few months are of significance to interventional pain physicians .
	manualset3
92459	1	399915	5	NULL	NULL	0	NULL	retinoic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , retinoic acid can activate ICD directly or through a Bmp-mediated mechanism .
	manualset3
92460	2	399915	5	NULL	NULL	0	NULL	ICD	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , retinoic acid can activate ICD directly or through a Bmp-mediated mechanism .
	manualset3
92461	3	399915	5	NULL	NULL	0	NULL	Bmp-mediated mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , retinoic acid can activate ICD directly or through a Bmp-mediated mechanism .
	manualset3
92462	1	399916	5	NULL	NULL	0	NULL	round to oval , eosinophilic , homogenous intracytoplasmic inclusions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , round to oval , eosinophilic , homogenous intracytoplasmic inclusions , several microm in average size , with a surrounding halo were found in the vast majority of hepatocytes .
	manualset3
92463	2	399916	5	NULL	NULL	0	NULL	several microm in average size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , round to oval , eosinophilic , homogenous intracytoplasmic inclusions , several microm in average size , with a surrounding halo were found in the vast majority of hepatocytes .
	manualset3
92464	3	399916	5	NULL	NULL	0	NULL	surrounding halo	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , round to oval , eosinophilic , homogenous intracytoplasmic inclusions , several microm in average size , with a surrounding halo were found in the vast majority of hepatocytes .
	manualset3
92465	4	399916	5	NULL	NULL	0	NULL	hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , round to oval , eosinophilic , homogenous intracytoplasmic inclusions , several microm in average size , with a surrounding halo were found in the vast majority of hepatocytes .
	manualset3
92467	1	399917	5	NULL	NULL	0	NULL	sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , sequence corresponding to the rotifer SL exon was found at the 5 ' - end of a number of full-length complementary DNA ( cDNA ) clones in a rice ( Oryza sativa ) database .
	manualset3
92468	2	399917	5	NULL	NULL	0	NULL	rotifer SL exon	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , sequence corresponding to the rotifer SL exon was found at the 5 ' - end of a number of full-length complementary DNA ( cDNA ) clones in a rice ( Oryza sativa ) database .
	manualset3
92469	3	399917	5	NULL	NULL	0	NULL	5 ' - end of a number of full-length complementary DNA ( cDNA ) clones	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , sequence corresponding to the rotifer SL exon was found at the 5 ' - end of a number of full-length complementary DNA ( cDNA ) clones in a rice ( Oryza sativa ) database .
	manualset3
92470	4	399917	5	NULL	NULL	0	NULL	rice ( Oryza sativa ) database	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , sequence corresponding to the rotifer SL exon was found at the 5 ' - end of a number of full-length complementary DNA ( cDNA ) clones in a rice ( Oryza sativa ) database .
	manualset3
92472	1	399918	5	NULL	NULL	0	NULL	LTP 1 function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , since LTP 1 function is regulated by the lipid content of plasma lipoproteins , we suggest that changes in lipoprotein composition that occur in dyslipidemia regulate the distribution of these and other hydrophobic drugs ( i.e. , annamycin and nystatin ) .
	manualset3
92473	2	399918	5	NULL	NULL	0	NULL	lipid content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , since LTP 1 function is regulated by the lipid content of plasma lipoproteins , we suggest that changes in lipoprotein composition that occur in dyslipidemia regulate the distribution of these and other hydrophobic drugs ( i.e. , annamycin and nystatin ) .
	manualset3
92474	3	399918	5	NULL	NULL	0	NULL	plasma lipoproteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , since LTP 1 function is regulated by the lipid content of plasma lipoproteins , we suggest that changes in lipoprotein composition that occur in dyslipidemia regulate the distribution of these and other hydrophobic drugs ( i.e. , annamycin and nystatin ) .
	manualset3
92475	4	399918	5	NULL	NULL	NULL	NULL	changes in lipoprotein composition	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , since LTP 1 function is regulated by the lipid content of plasma lipoproteins , we suggest that changes in lipoprotein composition that occur in dyslipidemia regulate the distribution of these and other hydrophobic drugs ( i.e. , annamycin and nystatin ) .
	manualset3
92476	5	399918	5	NULL	NULL	0	NULL	dyslipidemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , since LTP 1 function is regulated by the lipid content of plasma lipoproteins , we suggest that changes in lipoprotein composition that occur in dyslipidemia regulate the distribution of these and other hydrophobic drugs ( i.e. , annamycin and nystatin ) .
	manualset3
92477	6	399918	5	NULL	NULL	0	NULL	distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , since LTP 1 function is regulated by the lipid content of plasma lipoproteins , we suggest that changes in lipoprotein composition that occur in dyslipidemia regulate the distribution of these and other hydrophobic drugs ( i.e. , annamycin and nystatin ) .
	manualset3
92478	7	399918	5	NULL	NULL	0	NULL	hydrophobic drugs	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , since LTP 1 function is regulated by the lipid content of plasma lipoproteins , we suggest that changes in lipoprotein composition that occur in dyslipidemia regulate the distribution of these and other hydrophobic drugs ( i.e. , annamycin and nystatin ) .
	manualset3
92479	8	399918	5	NULL	NULL	0	NULL	annamycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , since LTP 1 function is regulated by the lipid content of plasma lipoproteins , we suggest that changes in lipoprotein composition that occur in dyslipidemia regulate the distribution of these and other hydrophobic drugs ( i.e. , annamycin and nystatin ) .
	manualset3
92480	9	399918	5	NULL	NULL	0	NULL	nystatin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , since LTP 1 function is regulated by the lipid content of plasma lipoproteins , we suggest that changes in lipoprotein composition that occur in dyslipidemia regulate the distribution of these and other hydrophobic drugs ( i.e. , annamycin and nystatin ) .
	manualset3
92481	1	399919	5	NULL	NULL	0	NULL	clusters	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , some clusters displayed patterns of activation that conveyed additional information necessary for successful performance of the task , such as the initial target velocity and the interval between successive submovements , suggesting that such information is represented in selective subpopulations of neurons in the primary motor cortex .
	manualset3
92482	2	399919	5	NULL	NULL	NULL	NULL	patterns of activation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , some clusters displayed patterns of activation that conveyed additional information necessary for successful performance of the task , such as the initial target velocity and the interval between successive submovements , suggesting that such information is represented in selective subpopulations of neurons in the primary motor cortex .
	manualset3
92562	3	399919	5	NULL	NULL	0	NULL	additional information	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , some clusters displayed patterns of activation that conveyed additional information necessary for successful performance of the task , such as the initial target velocity and the interval between successive submovements , suggesting that such information is represented in selective subpopulations of neurons in the primary motor cortex .
	manualset3
92563	4	399919	5	NULL	NULL	0	NULL	successful performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , some clusters displayed patterns of activation that conveyed additional information necessary for successful performance of the task , such as the initial target velocity and the interval between successive submovements , suggesting that such information is represented in selective subpopulations of neurons in the primary motor cortex .
	manualset3
92564	5	399919	5	NULL	NULL	0	NULL	task	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , some clusters displayed patterns of activation that conveyed additional information necessary for successful performance of the task , such as the initial target velocity and the interval between successive submovements , suggesting that such information is represented in selective subpopulations of neurons in the primary motor cortex .
	manualset3
92565	6	399919	5	NULL	NULL	0	NULL	initial target velocity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , some clusters displayed patterns of activation that conveyed additional information necessary for successful performance of the task , such as the initial target velocity and the interval between successive submovements , suggesting that such information is represented in selective subpopulations of neurons in the primary motor cortex .
	manualset3
92566	7	399919	5	NULL	NULL	0	NULL	interval between successive submovements	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , some clusters displayed patterns of activation that conveyed additional information necessary for successful performance of the task , such as the initial target velocity and the interval between successive submovements , suggesting that such information is represented in selective subpopulations of neurons in the primary motor cortex .
	manualset3
92567	8	399919	5	NULL	NULL	0	NULL	information	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , some clusters displayed patterns of activation that conveyed additional information necessary for successful performance of the task , such as the initial target velocity and the interval between successive submovements , suggesting that such information is represented in selective subpopulations of neurons in the primary motor cortex .
	manualset3
92568	9	399919	5	NULL	NULL	NULL	NULL	selective subpopulations of neurons	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , some clusters displayed patterns of activation that conveyed additional information necessary for successful performance of the task , such as the initial target velocity and the interval between successive submovements , suggesting that such information is represented in selective subpopulations of neurons in the primary motor cortex .
	manualset3
92570	10	399919	5	NULL	NULL	NULL	NULL	primary motor cortex	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , some clusters displayed patterns of activation that conveyed additional information necessary for successful performance of the task , such as the initial target velocity and the interval between successive submovements , suggesting that such information is represented in selective subpopulations of neurons in the primary motor cortex .
	manualset3
92483	1	399920	5	NULL	NULL	0	NULL	strong reactivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , strong reactivity was found in the circulating mononuclear cells of capsular blood vessels .
	manualset3
92484	2	399920	5	NULL	NULL	0	NULL	circulating mononuclear cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , strong reactivity was found in the circulating mononuclear cells of capsular blood vessels .
	manualset3
92485	3	399920	5	NULL	NULL	0	NULL	capsular blood vessels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , strong reactivity was found in the circulating mononuclear cells of capsular blood vessels .
	manualset3
92486	1	399921	5	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , studies are presented that have investigated the role of force feedback in surgical simulators .
	manualset3
92487	2	399921	5	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , studies are presented that have investigated the role of force feedback in surgical simulators .
	manualset3
92488	3	399921	5	NULL	NULL	0	NULL	force feedback	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , studies are presented that have investigated the role of force feedback in surgical simulators .
	manualset3
92489	4	399921	5	NULL	NULL	0	NULL	surgical simulators	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , studies are presented that have investigated the role of force feedback in surgical simulators .
	manualset3
92490	1	399922	5	NULL	NULL	0	NULL	study 2	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , study 2 revealed a significant time-by-phase interaction for glucose ( P = 0 .
	manualset3
92491	2	399922	5	NULL	NULL	0	NULL	significant time-by-phase interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , study 2 revealed a significant time-by-phase interaction for glucose ( P = 0 .
	manualset3
92492	3	399922	5	NULL	NULL	0	NULL	glucose	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , study 2 revealed a significant time-by-phase interaction for glucose ( P = 0 .
	manualset3
92493	4	399922	5	NULL	NULL	0	NULL	P = 0	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , study 2 revealed a significant time-by-phase interaction for glucose ( P = 0 .
	manualset3
92494	1	399923	5	NULL	NULL	0	NULL	continuous arterial infusion chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Usefulness of continuous arterial infusion chemotherapy for post operative multiple recurrence and residual hepatocellular carcinoma ) .
	manualset3
92495	2	399923	5	NULL	NULL	0	NULL	post operative multiple recurrence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Usefulness of continuous arterial infusion chemotherapy for post operative multiple recurrence and residual hepatocellular carcinoma ) .
	manualset3
92496	3	399923	5	NULL	NULL	0	NULL	residual hepatocellular carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Usefulness of continuous arterial infusion chemotherapy for post operative multiple recurrence and residual hepatocellular carcinoma ) .
	manualset3
92498	1	399924	5	NULL	NULL	0	NULL	successful therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , successful therapy normalized levels of mRNA for GATA-3 and Txk , although those for the others including IL-4 , IL-5 , IL-10 , IL-13 and IFN-gamma did not change .
	manualset3
92499	2	399924	5	NULL	NULL	0	NULL	levels of mRNA	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , successful therapy normalized levels of mRNA for GATA-3 and Txk , although those for the others including IL-4 , IL-5 , IL-10 , IL-13 and IFN-gamma did not change .
	manualset3
92500	3	399924	5	NULL	NULL	NULL	NULL	GATA-3	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , successful therapy normalized levels of mRNA for GATA-3 and Txk , although those for the others including IL-4 , IL-5 , IL-10 , IL-13 and IFN-gamma did not change .
	manualset3
92501	4	399924	5	NULL	NULL	NULL	NULL	Txk	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , successful therapy normalized levels of mRNA for GATA-3 and Txk , although those for the others including IL-4 , IL-5 , IL-10 , IL-13 and IFN-gamma did not change .
	manualset3
92503	5	399924	5	NULL	NULL	0	NULL	IL-4	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , successful therapy normalized levels of mRNA for GATA-3 and Txk , although those for the others including IL-4 , IL-5 , IL-10 , IL-13 and IFN-gamma did not change .
	manualset3
92504	6	399924	5	NULL	NULL	0	NULL	IL-5	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , successful therapy normalized levels of mRNA for GATA-3 and Txk , although those for the others including IL-4 , IL-5 , IL-10 , IL-13 and IFN-gamma did not change .
	manualset3
92505	7	399924	5	NULL	NULL	0	NULL	IL-10	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , successful therapy normalized levels of mRNA for GATA-3 and Txk , although those for the others including IL-4 , IL-5 , IL-10 , IL-13 and IFN-gamma did not change .
	manualset3
92506	8	399924	5	NULL	NULL	0	NULL	IL-13	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , successful therapy normalized levels of mRNA for GATA-3 and Txk , although those for the others including IL-4 , IL-5 , IL-10 , IL-13 and IFN-gamma did not change .
	manualset3
92507	9	399924	5	NULL	NULL	0	NULL	IFN-gamma	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , successful therapy normalized levels of mRNA for GATA-3 and Txk , although those for the others including IL-4 , IL-5 , IL-10 , IL-13 and IFN-gamma did not change .
	manualset3
92510	1	399925	5	NULL	NULL	NULL	NULL	terminal redundancy	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , terminal redundancy was observed as well as the presence of six tRNAs , one group I intron , and putative recombinases .
	manualset3
92511	2	399925	5	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , terminal redundancy was observed as well as the presence of six tRNAs , one group I intron , and putative recombinases .
	manualset3
92513	3	399925	5	NULL	NULL	0	NULL	six tRNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , terminal redundancy was observed as well as the presence of six tRNAs , one group I intron , and putative recombinases .
	manualset3
92514	4	399925	5	NULL	NULL	0	NULL	one group I intron	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , terminal redundancy was observed as well as the presence of six tRNAs , one group I intron , and putative recombinases .
	manualset3
92515	5	399925	5	NULL	NULL	0	NULL	putative recombinases	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , terminal redundancy was observed as well as the presence of six tRNAs , one group I intron , and putative recombinases .
	manualset3
92535	1	399926	5	NULL	NULL	NULL	NULL	HFrD	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , the HFrD blunted the increase in plasma NEFA and exogenous lipid oxidation during mental stress .
	manualset3
92536	2	399926	5	NULL	NULL	0	NULL	plasma NEFA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the HFrD blunted the increase in plasma NEFA and exogenous lipid oxidation during mental stress .
	manualset3
92537	3	399926	5	NULL	NULL	0	NULL	exogenous lipid oxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the HFrD blunted the increase in plasma NEFA and exogenous lipid oxidation during mental stress .
	manualset3
92538	4	399926	5	NULL	NULL	NULL	NULL	mental stress	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , the HFrD blunted the increase in plasma NEFA and exogenous lipid oxidation during mental stress .
	manualset3
92539	1	399927	5	NULL	NULL	0	NULL	analytical profile	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the analytical profile of 3-7 ring PNAs was of lower molecular weights in the coal treated with fuel oil .
	manualset3
92540	2	399927	5	NULL	NULL	0	NULL	3-7 ring PNAs	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the analytical profile of 3-7 ring PNAs was of lower molecular weights in the coal treated with fuel oil .
	manualset3
92541	3	399927	5	NULL	NULL	0	NULL	lower molecular weights	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the analytical profile of 3-7 ring PNAs was of lower molecular weights in the coal treated with fuel oil .
	manualset3
92542	4	399927	5	NULL	NULL	0	NULL	coal	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the analytical profile of 3-7 ring PNAs was of lower molecular weights in the coal treated with fuel oil .
	manualset3
92543	5	399927	5	NULL	NULL	0	NULL	fuel oil	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the analytical profile of 3-7 ring PNAs was of lower molecular weights in the coal treated with fuel oil .
	manualset3
92544	1	399928	5	NULL	NULL	0	NULL	basic principles	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the basic principles described in this manuscript apply to all liver-directed transarterial therapies , such as chemoembolization and/or drug-eluting microspheres .
	manualset3
92545	2	399928	5	NULL	NULL	0	NULL	manuscript	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the basic principles described in this manuscript apply to all liver-directed transarterial therapies , such as chemoembolization and/or drug-eluting microspheres .
	manualset3
92546	3	399928	5	NULL	NULL	0	NULL	liver-directed transarterial therapies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the basic principles described in this manuscript apply to all liver-directed transarterial therapies , such as chemoembolization and/or drug-eluting microspheres .
	manualset3
92547	4	399928	5	NULL	NULL	0	NULL	chemoembolization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the basic principles described in this manuscript apply to all liver-directed transarterial therapies , such as chemoembolization and/or drug-eluting microspheres .
	manualset3
92548	5	399928	5	NULL	NULL	0	NULL	drug-eluting microspheres	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the basic principles described in this manuscript apply to all liver-directed transarterial therapies , such as chemoembolization and/or drug-eluting microspheres .
	manualset3
92549	1	399929	5	NULL	NULL	0	NULL	chemotactic platelet adhesion-promoting substance leukotriene B4	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the chemotactic platelet adhesion-promoting substance leukotriene B4 is suppressed .
	manualset3
92550	1	399930	5	NULL	NULL	0	NULL	circulating B cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the circulating B cells expressed CD1c , CD38 , CD5 , and CD23 for the first year following transplant , antigens that are normally expressed on a small percentage of circulating B cells in normal adults , but highly expressed on cord blood B cells .
	manualset3
92551	2	399930	5	NULL	NULL	0	NULL	CD1c	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the circulating B cells expressed CD1c , CD38 , CD5 , and CD23 for the first year following transplant , antigens that are normally expressed on a small percentage of circulating B cells in normal adults , but highly expressed on cord blood B cells .
	manualset3
92552	3	399930	5	NULL	NULL	0	NULL	CD38	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the circulating B cells expressed CD1c , CD38 , CD5 , and CD23 for the first year following transplant , antigens that are normally expressed on a small percentage of circulating B cells in normal adults , but highly expressed on cord blood B cells .
	manualset3
92553	4	399930	5	NULL	NULL	0	NULL	CD5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the circulating B cells expressed CD1c , CD38 , CD5 , and CD23 for the first year following transplant , antigens that are normally expressed on a small percentage of circulating B cells in normal adults , but highly expressed on cord blood B cells .
	manualset3
92554	5	399930	5	NULL	NULL	0	NULL	CD23	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the circulating B cells expressed CD1c , CD38 , CD5 , and CD23 for the first year following transplant , antigens that are normally expressed on a small percentage of circulating B cells in normal adults , but highly expressed on cord blood B cells .
	manualset3
92555	6	399930	5	NULL	NULL	0	NULL	first year	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the circulating B cells expressed CD1c , CD38 , CD5 , and CD23 for the first year following transplant , antigens that are normally expressed on a small percentage of circulating B cells in normal adults , but highly expressed on cord blood B cells .
	manualset3
92556	7	399930	5	NULL	NULL	0	NULL	transplant	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the circulating B cells expressed CD1c , CD38 , CD5 , and CD23 for the first year following transplant , antigens that are normally expressed on a small percentage of circulating B cells in normal adults , but highly expressed on cord blood B cells .
	manualset3
92557	8	399930	5	NULL	NULL	0	NULL	antigens	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the circulating B cells expressed CD1c , CD38 , CD5 , and CD23 for the first year following transplant , antigens that are normally expressed on a small percentage of circulating B cells in normal adults , but highly expressed on cord blood B cells .
	manualset3
92558	9	399930	5	NULL	NULL	0	NULL	small percentage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the circulating B cells expressed CD1c , CD38 , CD5 , and CD23 for the first year following transplant , antigens that are normally expressed on a small percentage of circulating B cells in normal adults , but highly expressed on cord blood B cells .
	manualset3
92559	10	399930	5	NULL	NULL	0	NULL	circulating B cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the circulating B cells expressed CD1c , CD38 , CD5 , and CD23 for the first year following transplant , antigens that are normally expressed on a small percentage of circulating B cells in normal adults , but highly expressed on cord blood B cells .
	manualset3
92560	11	399930	5	NULL	NULL	0	NULL	normal adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the circulating B cells expressed CD1c , CD38 , CD5 , and CD23 for the first year following transplant , antigens that are normally expressed on a small percentage of circulating B cells in normal adults , but highly expressed on cord blood B cells .
	manualset3
92561	12	399930	5	NULL	NULL	0	NULL	cord blood B cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the circulating B cells expressed CD1c , CD38 , CD5 , and CD23 for the first year following transplant , antigens that are normally expressed on a small percentage of circulating B cells in normal adults , but highly expressed on cord blood B cells .
	manualset3
92572	1	399931	5	NULL	NULL	0	NULL	concentration-response curve	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the concentration-response curve of U46619 was shifted to the right after NQ12 treatment , indicating an antagonism on thromboxane ( TX ) A ( 2 ) receptors .
	manualset3
92573	2	399931	5	NULL	NULL	0	NULL	U46619	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the concentration-response curve of U46619 was shifted to the right after NQ12 treatment , indicating an antagonism on thromboxane ( TX ) A ( 2 ) receptors .
	manualset3
92574	3	399931	5	NULL	NULL	0	NULL	NQ12 treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the concentration-response curve of U46619 was shifted to the right after NQ12 treatment , indicating an antagonism on thromboxane ( TX ) A ( 2 ) receptors .
	manualset3
92575	4	399931	5	NULL	NULL	0	NULL	antagonism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the concentration-response curve of U46619 was shifted to the right after NQ12 treatment , indicating an antagonism on thromboxane ( TX ) A ( 2 ) receptors .
	manualset3
92576	5	399931	5	NULL	NULL	0	NULL	thromboxane ( TX ) A ( 2 ) receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the concentration-response curve of U46619 was shifted to the right after NQ12 treatment , indicating an antagonism on thromboxane ( TX ) A ( 2 ) receptors .
	manualset3
92785	1	399932	5	NULL	NULL	0	NULL	high-sensitivity CRP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Usefulness of high-sensitivity CRP increases during circadian rhythm for prediction of long-term cardiovascular events in patients with stable coronary artery disease ) .
	manualset3
92786	2	399932	5	NULL	NULL	0	NULL	circadian rhythm	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Usefulness of high-sensitivity CRP increases during circadian rhythm for prediction of long-term cardiovascular events in patients with stable coronary artery disease ) .
	manualset3
92787	3	399932	5	NULL	NULL	0	NULL	prediction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Usefulness of high-sensitivity CRP increases during circadian rhythm for prediction of long-term cardiovascular events in patients with stable coronary artery disease ) .
	manualset3
92788	4	399932	5	NULL	NULL	0	NULL	long-term cardiovascular events	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Usefulness of high-sensitivity CRP increases during circadian rhythm for prediction of long-term cardiovascular events in patients with stable coronary artery disease ) .
	manualset3
92789	5	399932	5	NULL	NULL	0	NULL	patients with stable coronary artery disease	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Usefulness of high-sensitivity CRP increases during circadian rhythm for prediction of long-term cardiovascular events in patients with stable coronary artery disease ) .
	manualset3
92790	1	399933	5	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the development of a thin collagenous internal capsule with endothelial cells secreting high levels of prostacyclin was observed at both anastomoses of the myxalin-treated grafts sterilized by gamma radiation .
	manualset3
92791	2	399933	5	NULL	NULL	0	NULL	thin collagenous internal capsule	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the development of a thin collagenous internal capsule with endothelial cells secreting high levels of prostacyclin was observed at both anastomoses of the myxalin-treated grafts sterilized by gamma radiation .
	manualset3
92792	3	399933	5	NULL	NULL	0	NULL	endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the development of a thin collagenous internal capsule with endothelial cells secreting high levels of prostacyclin was observed at both anastomoses of the myxalin-treated grafts sterilized by gamma radiation .
	manualset3
92793	4	399933	5	NULL	NULL	0	NULL	high levels of prostacyclin	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the development of a thin collagenous internal capsule with endothelial cells secreting high levels of prostacyclin was observed at both anastomoses of the myxalin-treated grafts sterilized by gamma radiation .
	manualset3
92798	5	399933	5	NULL	NULL	NULL	NULL	anastomoses of the myxalin-treated grafts	AnatomicalPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , the development of a thin collagenous internal capsule with endothelial cells secreting high levels of prostacyclin was observed at both anastomoses of the myxalin-treated grafts sterilized by gamma radiation .
	manualset3
92800	6	399933	5	NULL	NULL	0	NULL	gamma radiation	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the development of a thin collagenous internal capsule with endothelial cells secreting high levels of prostacyclin was observed at both anastomoses of the myxalin-treated grafts sterilized by gamma radiation .
	manualset3
92801	1	399934	5	NULL	NULL	0	NULL	double-strand-specific endoribonuclease III	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the double-strand-specific endoribonuclease III cleaves the two regions of the mRNA bound to RNAIII that may contribute to the degradation of the repressed mRNA .
	manualset3
92807	2	399934	5	NULL	NULL	0	NULL	two regions of the mRNA bound to RNAIII	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the double-strand-specific endoribonuclease III cleaves the two regions of the mRNA bound to RNAIII that may contribute to the degradation of the repressed mRNA .
	manualset3
92809	3	399934	5	NULL	NULL	0	NULL	degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the double-strand-specific endoribonuclease III cleaves the two regions of the mRNA bound to RNAIII that may contribute to the degradation of the repressed mRNA .
	manualset3
92810	4	399934	5	NULL	NULL	0	NULL	repressed mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the double-strand-specific endoribonuclease III cleaves the two regions of the mRNA bound to RNAIII that may contribute to the degradation of the repressed mRNA .
	manualset3
92959	1	399935	5	NULL	NULL	0	NULL	engagement of CD46-D2	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the engagement of CD46-D2 induces a conformational change in the DG loop in the Ad21 knob but not in the Ad11 knob .
	manualset3
92960	2	399935	5	NULL	NULL	0	NULL	conformational change	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the engagement of CD46-D2 induces a conformational change in the DG loop in the Ad21 knob but not in the Ad11 knob .
	manualset3
92961	3	399935	5	NULL	NULL	0	NULL	DG loop	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the engagement of CD46-D2 induces a conformational change in the DG loop in the Ad21 knob but not in the Ad11 knob .
	manualset3
92962	4	399935	5	NULL	NULL	0	NULL	Ad21 knob	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the engagement of CD46-D2 induces a conformational change in the DG loop in the Ad21 knob but not in the Ad11 knob .
	manualset3
92967	5	399935	5	NULL	NULL	0	NULL	Ad11 knob	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the engagement of CD46-D2 induces a conformational change in the DG loop in the Ad21 knob but not in the Ad11 knob .
	manualset3
92968	1	399936	5	NULL	NULL	0	NULL	expression of mutated PS1 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the expression of mutated PS1 elevated the level of phosphorylated beta-catenin , which is targeted to the ubiquitin/proteasome pathway .
	manualset3
92969	2	399936	5	NULL	NULL	0	NULL	level of phosphorylated beta-catenin	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the expression of mutated PS1 elevated the level of phosphorylated beta-catenin , which is targeted to the ubiquitin/proteasome pathway .
	manualset3
92970	3	399936	5	NULL	NULL	0	NULL	ubiquitin/proteasome pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the expression of mutated PS1 elevated the level of phosphorylated beta-catenin , which is targeted to the ubiquitin/proteasome pathway .
	manualset3
92971	1	399937	5	NULL	NULL	0	NULL	findings	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the findings show that , when instructions do not promote goal specificity , observation-based problem solving is as effective as action-based problem solving .
	manualset3
92972	2	399937	5	NULL	NULL	0	NULL	instructions	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the findings show that , when instructions do not promote goal specificity , observation-based problem solving is as effective as action-based problem solving .
	manualset3
92973	3	399937	5	NULL	NULL	0	NULL	goal specificity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the findings show that , when instructions do not promote goal specificity , observation-based problem solving is as effective as action-based problem solving .
	manualset3
92974	4	399937	5	NULL	NULL	0	NULL	observation-based problem solving	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the findings show that , when instructions do not promote goal specificity , observation-based problem solving is as effective as action-based problem solving .
	manualset3
92975	5	399937	5	NULL	NULL	0	NULL	action-based problem solving	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the findings show that , when instructions do not promote goal specificity , observation-based problem solving is as effective as action-based problem solving .
	manualset3
93003	1	399938	5	NULL	NULL	0	NULL	gradient watershed region hierarchy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the gradient watershed region hierarchy can be used for automatic or interactive image segmentation .
	manualset3
93004	2	399938	5	NULL	NULL	0	NULL	automatic or interactive image segmentation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the gradient watershed region hierarchy can be used for automatic or interactive image segmentation .
	manualset3
93005	1	399939	5	NULL	NULL	0	NULL	high dose of VIP	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the high dose of VIP and PHM transiently increased wakefulness .
	manualset3
93006	2	399939	5	NULL	NULL	0	NULL	high dose of PHM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the high dose of VIP and PHM transiently increased wakefulness .
	manualset3
93007	3	399939	5	NULL	NULL	NULL	NULL	wakefulness	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , the high dose of VIP and PHM transiently increased wakefulness .
	manualset3
93008	1	399940	5	NULL	NULL	0	NULL	hirudin54-65 peptide	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the hirudin54-65 peptide competed at submicromolar concentrations for the binding of alpha - and DIP-alpha-thrombin , but not for beta-thrombin .
	manualset3
93009	2	399940	5	NULL	NULL	0	NULL	submicromolar concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the hirudin54-65 peptide competed at submicromolar concentrations for the binding of alpha - and DIP-alpha-thrombin , but not for beta-thrombin .
	manualset3
93010	3	399940	5	NULL	NULL	0	NULL	alpha-thrombin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the hirudin54-65 peptide competed at submicromolar concentrations for the binding of alpha - and DIP-alpha-thrombin , but not for beta-thrombin .
	manualset3
93011	4	399940	5	NULL	NULL	0	NULL	DIP-alpha-thrombin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the hirudin54-65 peptide competed at submicromolar concentrations for the binding of alpha - and DIP-alpha-thrombin , but not for beta-thrombin .
	manualset3
93012	5	399940	5	NULL	NULL	0	NULL	beta-thrombin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the hirudin54-65 peptide competed at submicromolar concentrations for the binding of alpha - and DIP-alpha-thrombin , but not for beta-thrombin .
	manualset3
93013	1	399941	5	NULL	NULL	0	NULL	inhibitory effects of memantine	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the inhibitory effects of memantine on the expression of morphine-induced conditioned place preference seemed not to be related to effects on memory retrieval , as revealed in the Morris water maze spatial task .
	manualset3
93014	2	399941	5	NULL	NULL	0	NULL	expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the inhibitory effects of memantine on the expression of morphine-induced conditioned place preference seemed not to be related to effects on memory retrieval , as revealed in the Morris water maze spatial task .
	manualset3
93015	3	399941	5	NULL	NULL	0	NULL	morphine-induced conditioned place preference	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the inhibitory effects of memantine on the expression of morphine-induced conditioned place preference seemed not to be related to effects on memory retrieval , as revealed in the Morris water maze spatial task .
	manualset3
93016	4	399941	5	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the inhibitory effects of memantine on the expression of morphine-induced conditioned place preference seemed not to be related to effects on memory retrieval , as revealed in the Morris water maze spatial task .
	manualset3
93017	5	399941	5	NULL	NULL	0	NULL	memory retrieval	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the inhibitory effects of memantine on the expression of morphine-induced conditioned place preference seemed not to be related to effects on memory retrieval , as revealed in the Morris water maze spatial task .
	manualset3
93018	6	399941	5	NULL	NULL	0	NULL	Morris water maze spatial task	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the inhibitory effects of memantine on the expression of morphine-induced conditioned place preference seemed not to be related to effects on memory retrieval , as revealed in the Morris water maze spatial task .
	manualset3
93019	2	399942	5	NULL	NULL	NULL	NULL	patient care	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , the intensity of patient care could be considerably reduced .
	manualset3
93287	1	399942	5	NULL	NULL	0	NULL	intensity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the intensity of patient care could be considerably reduced .
	manualset3
93288	1	399943	5	NULL	NULL	0	NULL	PET/CT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Utility of PET/CT for mediastinal staging of non-small cell lung cancer in stage III ( N2 ) ) .
	manualset3
93289	2	399943	5	NULL	NULL	0	NULL	mediastinal staging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Utility of PET/CT for mediastinal staging of non-small cell lung cancer in stage III ( N2 ) ) .
	manualset3
93290	3	399943	5	NULL	NULL	NULL	NULL	non-small cell lung cancer in stage III ( N2 )	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Utility of PET/CT for mediastinal staging of non-small cell lung cancer in stage III ( N2 ) ) .
	manualset3
93291	1	399944	5	NULL	NULL	0	NULL	intestinal microbiota	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the intestinal microbiota plays a critical role in controlling Salmonella infection , disease , and transmissibility .
	manualset3
93292	2	399944	5	NULL	NULL	0	NULL	critical role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the intestinal microbiota plays a critical role in controlling Salmonella infection , disease , and transmissibility .
	manualset3
93293	3	399944	5	NULL	NULL	0	NULL	Salmonella infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the intestinal microbiota plays a critical role in controlling Salmonella infection , disease , and transmissibility .
	manualset3
93294	4	399944	5	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the intestinal microbiota plays a critical role in controlling Salmonella infection , disease , and transmissibility .
	manualset3
93295	1	399945	5	NULL	NULL	0	NULL	introduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the introduction of large micro-size cube phosphors can reduce the wide variation in optical properties as a function of both the ambient temperature and applied current compared with those of conventional powder phosphor-based white LEDs .
	manualset3
93296	2	399945	5	NULL	NULL	0	NULL	large micro-size cube phosphors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the introduction of large micro-size cube phosphors can reduce the wide variation in optical properties as a function of both the ambient temperature and applied current compared with those of conventional powder phosphor-based white LEDs .
	manualset3
93297	3	399945	5	NULL	NULL	0	NULL	wide variation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the introduction of large micro-size cube phosphors can reduce the wide variation in optical properties as a function of both the ambient temperature and applied current compared with those of conventional powder phosphor-based white LEDs .
	manualset3
93298	4	399945	5	NULL	NULL	0	NULL	optical properties	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the introduction of large micro-size cube phosphors can reduce the wide variation in optical properties as a function of both the ambient temperature and applied current compared with those of conventional powder phosphor-based white LEDs .
	manualset3
93299	5	399945	5	NULL	NULL	0	NULL	function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the introduction of large micro-size cube phosphors can reduce the wide variation in optical properties as a function of both the ambient temperature and applied current compared with those of conventional powder phosphor-based white LEDs .
	manualset3
93300	6	399945	5	NULL	NULL	0	NULL	ambient temperature	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the introduction of large micro-size cube phosphors can reduce the wide variation in optical properties as a function of both the ambient temperature and applied current compared with those of conventional powder phosphor-based white LEDs .
	manualset3
93301	7	399945	5	NULL	NULL	0	NULL	applied current	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the introduction of large micro-size cube phosphors can reduce the wide variation in optical properties as a function of both the ambient temperature and applied current compared with those of conventional powder phosphor-based white LEDs .
	manualset3
93302	8	399945	5	NULL	NULL	0	NULL	conventional powder phosphor-based white LEDs	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the introduction of large micro-size cube phosphors can reduce the wide variation in optical properties as a function of both the ambient temperature and applied current compared with those of conventional powder phosphor-based white LEDs .
	manualset3
93303	1	399946	5	NULL	NULL	0	NULL	novel compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the novel compounds also found in this search are promising therapeutic agents that could beneficially affect feeding behavior .
	manualset3
93304	2	399946	5	NULL	NULL	0	NULL	search	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the novel compounds also found in this search are promising therapeutic agents that could beneficially affect feeding behavior .
	manualset3
93305	3	399946	5	NULL	NULL	0	NULL	promising therapeutic agents 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the novel compounds also found in this search are promising therapeutic agents that could beneficially affect feeding behavior .
	manualset3
93307	4	399946	5	NULL	NULL	NULL	NULL	feeding behavior	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , the novel compounds also found in this search are promising therapeutic agents that could beneficially affect feeding behavior .
	manualset3
93308	1	399947	5	NULL	NULL	0	NULL	overexpression	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the overexpression of ATF6 increased the Oc promoter activity by enhancing the direct binding to a putative ATF6 binding motif ( TGACGT , -1126 to -1121 bp ) .
	manualset3
93309	2	399947	5	NULL	NULL	0	NULL	ATF6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the overexpression of ATF6 increased the Oc promoter activity by enhancing the direct binding to a putative ATF6 binding motif ( TGACGT , -1126 to -1121 bp ) .
	manualset3
93310	3	399947	5	NULL	NULL	0	NULL	Oc promoter activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the overexpression of ATF6 increased the Oc promoter activity by enhancing the direct binding to a putative ATF6 binding motif ( TGACGT , -1126 to -1121 bp ) .
	manualset3
93311	4	399947	5	NULL	NULL	0	NULL	putative ATF6 binding motif ( TGACGT , -1126 to -1121 bp )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the overexpression of ATF6 increased the Oc promoter activity by enhancing the direct binding to a putative ATF6 binding motif ( TGACGT , -1126 to -1121 bp ) .
	manualset3
98563	5	399947	5	NULL	NULL	0	NULL	direct binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the overexpression of ATF6 increased the Oc promoter activity by enhancing the direct binding to a putative ATF6 binding motif ( TGACGT , -1126 to -1121 bp ) .
	manualset3
93312	1	399948	5	NULL	NULL	0	NULL	predicted amino-terminal sequences	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the predicted amino-terminal sequences of I. scapularis MPs were found by Edman degradation of PVDF-transferred SDS/PAGE-separated tick saliva proteins , indicating that these putative enzymes are secreted .
	manualset3
93313	2	399948	5	NULL	NULL	0	NULL	I. scapularis MPs	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the predicted amino-terminal sequences of I. scapularis MPs were found by Edman degradation of PVDF-transferred SDS/PAGE-separated tick saliva proteins , indicating that these putative enzymes are secreted .
	manualset3
93314	3	399948	5	NULL	NULL	0	NULL	Edman degradation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the predicted amino-terminal sequences of I. scapularis MPs were found by Edman degradation of PVDF-transferred SDS/PAGE-separated tick saliva proteins , indicating that these putative enzymes are secreted .
	manualset3
93315	4	399948	5	NULL	NULL	0	NULL	PVDF-transferred SDS/PAGE-separated tick saliva proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the predicted amino-terminal sequences of I. scapularis MPs were found by Edman degradation of PVDF-transferred SDS/PAGE-separated tick saliva proteins , indicating that these putative enzymes are secreted .
	manualset3
93316	5	399948	5	NULL	NULL	0	NULL	putative enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the predicted amino-terminal sequences of I. scapularis MPs were found by Edman degradation of PVDF-transferred SDS/PAGE-separated tick saliva proteins , indicating that these putative enzymes are secreted .
	manualset3
93317	1	399949	5	NULL	NULL	0	NULL	proteasome inhibitor Bortezomib	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the proteasome inhibitor Bortezomib , which is described to antagonize NF-B activity , had a consistent antitumor activity against both chemoresistant and chemosensitive MM-cells , regardless the NF-B localization , thus suggesting the existence of other molecular targets of proteasome inhibitors in MM .
	manualset3
93318	2	399949	5	NULL	NULL	0	NULL	NF-B activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the proteasome inhibitor Bortezomib , which is described to antagonize NF-B activity , had a consistent antitumor activity against both chemoresistant and chemosensitive MM-cells , regardless the NF-B localization , thus suggesting the existence of other molecular targets of proteasome inhibitors in MM .
	manualset3
93319	3	399949	5	NULL	NULL	0	NULL	consistent antitumor activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the proteasome inhibitor Bortezomib , which is described to antagonize NF-B activity , had a consistent antitumor activity against both chemoresistant and chemosensitive MM-cells , regardless the NF-B localization , thus suggesting the existence of other molecular targets of proteasome inhibitors in MM .
	manualset3
93320	4	399949	5	NULL	NULL	0	NULL	chemoresistant MM-cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the proteasome inhibitor Bortezomib , which is described to antagonize NF-B activity , had a consistent antitumor activity against both chemoresistant and chemosensitive MM-cells , regardless the NF-B localization , thus suggesting the existence of other molecular targets of proteasome inhibitors in MM .
	manualset3
93321	5	399949	5	NULL	NULL	0	NULL	chemosensitive MM-cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the proteasome inhibitor Bortezomib , which is described to antagonize NF-B activity , had a consistent antitumor activity against both chemoresistant and chemosensitive MM-cells , regardless the NF-B localization , thus suggesting the existence of other molecular targets of proteasome inhibitors in MM .
	manualset3
93322	6	399949	5	NULL	NULL	0	NULL	NF-B localization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the proteasome inhibitor Bortezomib , which is described to antagonize NF-B activity , had a consistent antitumor activity against both chemoresistant and chemosensitive MM-cells , regardless the NF-B localization , thus suggesting the existence of other molecular targets of proteasome inhibitors in MM .
	manualset3
93323	7	399949	5	NULL	NULL	0	NULL	existence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the proteasome inhibitor Bortezomib , which is described to antagonize NF-B activity , had a consistent antitumor activity against both chemoresistant and chemosensitive MM-cells , regardless the NF-B localization , thus suggesting the existence of other molecular targets of proteasome inhibitors in MM .
	manualset3
93324	8	399949	5	NULL	NULL	0	NULL	molecular targets of proteasome inhibitors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the proteasome inhibitor Bortezomib , which is described to antagonize NF-B activity , had a consistent antitumor activity against both chemoresistant and chemosensitive MM-cells , regardless the NF-B localization , thus suggesting the existence of other molecular targets of proteasome inhibitors in MM .
	manualset3
93325	9	399949	5	NULL	NULL	0	NULL	MM	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the proteasome inhibitor Bortezomib , which is described to antagonize NF-B activity , had a consistent antitumor activity against both chemoresistant and chemosensitive MM-cells , regardless the NF-B localization , thus suggesting the existence of other molecular targets of proteasome inhibitors in MM .
	manualset3
93326	1	399950	5	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the recent development of novel approaches such as neoadjuvant tumor therapy , cryosurgery , thermal ablative techniques as well as biological and immunological manipulation of malignant cells has added to the complexity of this field .
	manualset3
93327	2	399950	5	NULL	NULL	0	NULL	novel approaches	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the recent development of novel approaches such as neoadjuvant tumor therapy , cryosurgery , thermal ablative techniques as well as biological and immunological manipulation of malignant cells has added to the complexity of this field .
	manualset3
93328	3	399950	5	NULL	NULL	0	NULL	neoadjuvant tumor therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the recent development of novel approaches such as neoadjuvant tumor therapy , cryosurgery , thermal ablative techniques as well as biological and immunological manipulation of malignant cells has added to the complexity of this field .
	manualset3
93329	4	399950	5	NULL	NULL	0	NULL	cryosurgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the recent development of novel approaches such as neoadjuvant tumor therapy , cryosurgery , thermal ablative techniques as well as biological and immunological manipulation of malignant cells has added to the complexity of this field .
	manualset3
93330	5	399950	5	NULL	NULL	0	NULL	thermal ablative techniques	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the recent development of novel approaches such as neoadjuvant tumor therapy , cryosurgery , thermal ablative techniques as well as biological and immunological manipulation of malignant cells has added to the complexity of this field .
	manualset3
93331	6	399950	5	NULL	NULL	0	NULL	biological and immunological manipulation of malignant cells	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the recent development of novel approaches such as neoadjuvant tumor therapy , cryosurgery , thermal ablative techniques as well as biological and immunological manipulation of malignant cells has added to the complexity of this field .
	manualset3
93332	7	399950	5	NULL	NULL	0	NULL	complexity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the recent development of novel approaches such as neoadjuvant tumor therapy , cryosurgery , thermal ablative techniques as well as biological and immunological manipulation of malignant cells has added to the complexity of this field .
	manualset3
93333	1	399951	5	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the relation between childhood healthcare experience and current healthcare behavior was moderated by optimism , such that those who reported both more negative childhood healthcare experiences and low levels of optimism reported the least adaptive healthcare behaviors and those who reported the most positive childhood healthcare experience and the highest levels of optimism reported the most adaptive healthcare behavior .
	manualset3
93334	2	399951	5	NULL	NULL	0	NULL	childhood healthcare experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the relation between childhood healthcare experience and current healthcare behavior was moderated by optimism , such that those who reported both more negative childhood healthcare experiences and low levels of optimism reported the least adaptive healthcare behaviors and those who reported the most positive childhood healthcare experience and the highest levels of optimism reported the most adaptive healthcare behavior .
	manualset3
93335	3	399951	5	NULL	NULL	0	NULL	current healthcare behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the relation between childhood healthcare experience and current healthcare behavior was moderated by optimism , such that those who reported both more negative childhood healthcare experiences and low levels of optimism reported the least adaptive healthcare behaviors and those who reported the most positive childhood healthcare experience and the highest levels of optimism reported the most adaptive healthcare behavior .
	manualset3
93527	4	399951	5	NULL	NULL	0	NULL	optimism	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the relation between childhood healthcare experience and current healthcare behavior was moderated by optimism , such that those who reported both more negative childhood healthcare experiences and low levels of optimism reported the least adaptive healthcare behaviors and those who reported the most positive childhood healthcare experience and the highest levels of optimism reported the most adaptive healthcare behavior .
	manualset3
93528	5	399951	5	NULL	NULL	0	NULL	negative childhood healthcare experiences	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the relation between childhood healthcare experience and current healthcare behavior was moderated by optimism , such that those who reported both more negative childhood healthcare experiences and low levels of optimism reported the least adaptive healthcare behaviors and those who reported the most positive childhood healthcare experience and the highest levels of optimism reported the most adaptive healthcare behavior .
	manualset3
93529	6	399951	5	NULL	NULL	0	NULL	low levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the relation between childhood healthcare experience and current healthcare behavior was moderated by optimism , such that those who reported both more negative childhood healthcare experiences and low levels of optimism reported the least adaptive healthcare behaviors and those who reported the most positive childhood healthcare experience and the highest levels of optimism reported the most adaptive healthcare behavior .
	manualset3
93530	7	399951	5	NULL	NULL	0	NULL	optimism	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the relation between childhood healthcare experience and current healthcare behavior was moderated by optimism , such that those who reported both more negative childhood healthcare experiences and low levels of optimism reported the least adaptive healthcare behaviors and those who reported the most positive childhood healthcare experience and the highest levels of optimism reported the most adaptive healthcare behavior .
	manualset3
93531	8	399951	5	NULL	NULL	0	NULL	least adaptive healthcare behaviors	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the relation between childhood healthcare experience and current healthcare behavior was moderated by optimism , such that those who reported both more negative childhood healthcare experiences and low levels of optimism reported the least adaptive healthcare behaviors and those who reported the most positive childhood healthcare experience and the highest levels of optimism reported the most adaptive healthcare behavior .
	manualset3
93532	9	399951	5	NULL	NULL	0	NULL	most positive childhood healthcare experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the relation between childhood healthcare experience and current healthcare behavior was moderated by optimism , such that those who reported both more negative childhood healthcare experiences and low levels of optimism reported the least adaptive healthcare behaviors and those who reported the most positive childhood healthcare experience and the highest levels of optimism reported the most adaptive healthcare behavior .
	manualset3
93533	10	399951	5	NULL	NULL	0	NULL	highest levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the relation between childhood healthcare experience and current healthcare behavior was moderated by optimism , such that those who reported both more negative childhood healthcare experiences and low levels of optimism reported the least adaptive healthcare behaviors and those who reported the most positive childhood healthcare experience and the highest levels of optimism reported the most adaptive healthcare behavior .
	manualset3
93534	11	399951	5	NULL	NULL	0	NULL	optimism	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the relation between childhood healthcare experience and current healthcare behavior was moderated by optimism , such that those who reported both more negative childhood healthcare experiences and low levels of optimism reported the least adaptive healthcare behaviors and those who reported the most positive childhood healthcare experience and the highest levels of optimism reported the most adaptive healthcare behavior .
	manualset3
93535	12	399951	5	NULL	NULL	0	NULL	most adaptive healthcare behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the relation between childhood healthcare experience and current healthcare behavior was moderated by optimism , such that those who reported both more negative childhood healthcare experiences and low levels of optimism reported the least adaptive healthcare behaviors and those who reported the most positive childhood healthcare experience and the highest levels of optimism reported the most adaptive healthcare behavior .
	manualset3
93536	1	399952	5	NULL	NULL	0	NULL	transparietal cholangiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Utility of transparietal cholangiography in the diagnosis of jaundice ) .
	manualset3
93537	2	399952	5	NULL	NULL	0	NULL	jaundice	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Utility of transparietal cholangiography in the diagnosis of jaundice ) .
	manualset3
98564	3	399952	5	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Utility of transparietal cholangiography in the diagnosis of jaundice ) .
	manualset3
93538	1	399953	5	NULL	NULL	0	NULL	death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the underlying cause of death that originally was manually classified for the official mortality statistics was retrieved from Statistics Norway in all cases .
	manualset3
93539	2	399953	5	NULL	NULL	0	NULL	official mortality statistics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the underlying cause of death that originally was manually classified for the official mortality statistics was retrieved from Statistics Norway in all cases .
	manualset3
93540	3	399953	5	NULL	NULL	0	NULL	Statistics Norway	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the underlying cause of death that originally was manually classified for the official mortality statistics was retrieved from Statistics Norway in all cases .
	manualset3
93541	4	399953	5	NULL	NULL	NULL	NULL	cases	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , the underlying cause of death that originally was manually classified for the official mortality statistics was retrieved from Statistics Norway in all cases .
	manualset3
98565	5	399953	5	NULL	NULL	0	NULL	cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the underlying cause of death that originally was manually classified for the official mortality statistics was retrieved from Statistics Norway in all cases .
	manualset3
93542	1	399954	5	NULL	NULL	0	NULL	vault protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the vault protein localizes to short linear strings juxtaposed to the exterior of the nucleus and extending outward into the cytoplasm .
	manualset3
93543	2	399954	5	NULL	NULL	0	NULL	short linear strings	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the vault protein localizes to short linear strings juxtaposed to the exterior of the nucleus and extending outward into the cytoplasm .
	manualset3
93544	3	399954	5	NULL	NULL	0	NULL	nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the vault protein localizes to short linear strings juxtaposed to the exterior of the nucleus and extending outward into the cytoplasm .
	manualset3
93545	4	399954	5	NULL	NULL	0	NULL	cytoplasm	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the vault protein localizes to short linear strings juxtaposed to the exterior of the nucleus and extending outward into the cytoplasm .
	manualset3
93546	1	399955	5	NULL	NULL	0	NULL	increased trend	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , there was an increased trend ( P & lt ; 0.001 ) for right-sided ( from cecum to and including the splenic flexure ) CRC in patients both 50-74 and more than 75 years old .
	manualset3
93547	2	399955	5	NULL	NULL	0	NULL	P & lt ; 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , there was an increased trend ( P & lt ; 0.001 ) for right-sided ( from cecum to and including the splenic flexure ) CRC in patients both 50-74 and more than 75 years old .
	manualset3
93548	3	399955	5	NULL	NULL	0	NULL	cecum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , there was an increased trend ( P & lt ; 0.001 ) for right-sided ( from cecum to and including the splenic flexure ) CRC in patients both 50-74 and more than 75 years old .
	manualset3
93549	4	399955	5	NULL	NULL	0	NULL	splenic flexure	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , there was an increased trend ( P & lt ; 0.001 ) for right-sided ( from cecum to and including the splenic flexure ) CRC in patients both 50-74 and more than 75 years old .
	manualset3
93550	5	399955	5	NULL	NULL	0	NULL	right-sided CRC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , there was an increased trend ( P & lt ; 0.001 ) for right-sided ( from cecum to and including the splenic flexure ) CRC in patients both 50-74 and more than 75 years old .
	manualset3
93551	6	399955	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , there was an increased trend ( P & lt ; 0.001 ) for right-sided ( from cecum to and including the splenic flexure ) CRC in patients both 50-74 and more than 75 years old .
	manualset3
93552	7	399955	5	NULL	NULL	0	NULL	50-74	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , there was an increased trend ( P & lt ; 0.001 ) for right-sided ( from cecum to and including the splenic flexure ) CRC in patients both 50-74 and more than 75 years old .
	manualset3
93553	8	399955	5	NULL	NULL	0	NULL	more than 75 years old	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , there was an increased trend ( P & lt ; 0.001 ) for right-sided ( from cecum to and including the splenic flexure ) CRC in patients both 50-74 and more than 75 years old .
	manualset3
93554	1	399956	5	NULL	NULL	NULL	NULL	idea	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , they support the idea that efficient restoration of language is achieved if a sufficiently large neuronal network is preserved around the lesion .
	manualset3
93555	2	399956	5	NULL	NULL	0	NULL	efficient restoration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , they support the idea that efficient restoration of language is achieved if a sufficiently large neuronal network is preserved around the lesion .
	manualset3
93556	3	399956	5	NULL	NULL	0	NULL	language	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , they support the idea that efficient restoration of language is achieved if a sufficiently large neuronal network is preserved around the lesion .
	manualset3
93557	4	399956	5	NULL	NULL	0	NULL	sufficiently large neuronal network	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , they support the idea that efficient restoration of language is achieved if a sufficiently large neuronal network is preserved around the lesion .
	manualset3
93558	5	399956	5	NULL	NULL	0	NULL	lesion	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , they support the idea that efficient restoration of language is achieved if a sufficiently large neuronal network is preserved around the lesion .
	manualset3
93559	1	399957	5	NULL	NULL	0	NULL	tissue inhibitor of metalloproteinase-2 ( TIMP-2 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , tissue inhibitor of metalloproteinase-2 ( TIMP-2 ) attenuated Ihh-stimulated PSC migration .
	manualset3
93560	2	399957	5	NULL	NULL	0	NULL	Ihh-stimulated PSC migration	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , tissue inhibitor of metalloproteinase-2 ( TIMP-2 ) attenuated Ihh-stimulated PSC migration .
	manualset3
93561	1	399958	5	NULL	NULL	NULL	NULL	treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , treatment with anti-IL-17A antibody neutralizes IL-17A-mediated effects on adipocyte differentiation and function .
	manualset3
93562	2	399958	5	NULL	NULL	0	NULL	anti-IL-17A antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , treatment with anti-IL-17A antibody neutralizes IL-17A-mediated effects on adipocyte differentiation and function .
	manualset3
93563	3	399958	5	NULL	NULL	0	NULL	IL-17A-mediated effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , treatment with anti-IL-17A antibody neutralizes IL-17A-mediated effects on adipocyte differentiation and function .
	manualset3
93564	4	399958	5	NULL	NULL	0	NULL	adipocyte differentiation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , treatment with anti-IL-17A antibody neutralizes IL-17A-mediated effects on adipocyte differentiation and function .
	manualset3
93565	5	399958	5	NULL	NULL	0	NULL	function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , treatment with anti-IL-17A antibody neutralizes IL-17A-mediated effects on adipocyte differentiation and function .
	manualset3
93566	1	399959	5	NULL	NULL	0	NULL	32	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we also discovered 32 new miRNAs in the seedlings of rice .
	manualset3
93567	2	399959	5	NULL	NULL	0	NULL	miRNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we also discovered 32 new miRNAs in the seedlings of rice .
	manualset3
93568	3	399959	5	NULL	NULL	NULL	NULL	seedlings of rice	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , we also discovered 32 new miRNAs in the seedlings of rice .
	manualset3
93569	1	399960	5	NULL	NULL	0	NULL	distinct distribution patterns	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we also have noted the distinct distribution patterns of human loricrin and involucrin , another major precursor protein of the cornified cell envelope .
	manualset3
93570	2	399960	5	NULL	NULL	0	NULL	human loricrin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we also have noted the distinct distribution patterns of human loricrin and involucrin , another major precursor protein of the cornified cell envelope .
	manualset3
93571	3	399960	5	NULL	NULL	0	NULL	human involucrin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we also have noted the distinct distribution patterns of human loricrin and involucrin , another major precursor protein of the cornified cell envelope .
	manualset3
93572	4	399960	5	NULL	NULL	0	NULL	major precursor protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we also have noted the distinct distribution patterns of human loricrin and involucrin , another major precursor protein of the cornified cell envelope .
	manualset3
93573	5	399960	5	NULL	NULL	0	NULL	cornified cell envelope	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we also have noted the distinct distribution patterns of human loricrin and involucrin , another major precursor protein of the cornified cell envelope .
	manualset3
93574	1	399961	5	NULL	NULL	0	NULL	self-assembly	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we also investigate the self-assembly of diblock copolymers with different tails in a slit .
	manualset3
93575	2	399961	5	NULL	NULL	0	NULL	diblock copolymers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we also investigate the self-assembly of diblock copolymers with different tails in a slit .
	manualset3
93576	3	399961	5	NULL	NULL	0	NULL	different tails	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we also investigate the self-assembly of diblock copolymers with different tails in a slit .
	manualset3
93577	4	399961	5	NULL	NULL	0	NULL	slit	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we also investigate the self-assembly of diblock copolymers with different tails in a slit .
	manualset3
93578	1	399962	5	NULL	NULL	0	NULL	Pax2 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we assayed for Pax2 expression in glial cells in mammalian retinas .
	manualset3
93579	2	399962	5	NULL	NULL	0	NULL	glial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we assayed for Pax2 expression in glial cells in mammalian retinas .
	manualset3
93580	3	399962	5	NULL	NULL	0	NULL	mammalian retinas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we assayed for Pax2 expression in glial cells in mammalian retinas .
	manualset3
93581	1	399963	5	NULL	NULL	0	NULL	dysadherin mRNA expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we compared dysadherin mRNA expression between epithelioid sarcoma and malignant rhabdoid tumor cell lines , using RT-PCR and real-time quantitative RT-PCR analysis .
	manualset3
93582	2	399963	5	NULL	NULL	0	NULL	epithelioid sarcoma cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we compared dysadherin mRNA expression between epithelioid sarcoma and malignant rhabdoid tumor cell lines , using RT-PCR and real-time quantitative RT-PCR analysis .
	manualset3
93583	3	399963	5	NULL	NULL	0	NULL	malignant rhabdoid tumor cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we compared dysadherin mRNA expression between epithelioid sarcoma and malignant rhabdoid tumor cell lines , using RT-PCR and real-time quantitative RT-PCR analysis .
	manualset3
93584	4	399963	5	NULL	NULL	0	NULL	RT-PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we compared dysadherin mRNA expression between epithelioid sarcoma and malignant rhabdoid tumor cell lines , using RT-PCR and real-time quantitative RT-PCR analysis .
	manualset3
93585	5	399963	5	NULL	NULL	0	NULL	real-time quantitative RT-PCR analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we compared dysadherin mRNA expression between epithelioid sarcoma and malignant rhabdoid tumor cell lines , using RT-PCR and real-time quantitative RT-PCR analysis .
	manualset3
93586	1	399964	5	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we construct a model for the acquired multiunit signal drawing on basic assumptions regarding the nature of a single neuron , which explains the second-order statistics of the raw electrode voltage measurements that are high-pass-filtered above 300 Hz .
	manualset3
93587	2	399964	5	NULL	NULL	0	NULL	acquired multiunit signal drawing	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we construct a model for the acquired multiunit signal drawing on basic assumptions regarding the nature of a single neuron , which explains the second-order statistics of the raw electrode voltage measurements that are high-pass-filtered above 300 Hz .
	manualset3
93588	3	399964	5	NULL	NULL	0	NULL	basic assumptions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we construct a model for the acquired multiunit signal drawing on basic assumptions regarding the nature of a single neuron , which explains the second-order statistics of the raw electrode voltage measurements that are high-pass-filtered above 300 Hz .
	manualset3
93589	4	399964	5	NULL	NULL	0	NULL	nature	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we construct a model for the acquired multiunit signal drawing on basic assumptions regarding the nature of a single neuron , which explains the second-order statistics of the raw electrode voltage measurements that are high-pass-filtered above 300 Hz .
	manualset3
93590	5	399964	5	NULL	NULL	0	NULL	single neuron	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we construct a model for the acquired multiunit signal drawing on basic assumptions regarding the nature of a single neuron , which explains the second-order statistics of the raw electrode voltage measurements that are high-pass-filtered above 300 Hz .
	manualset3
93591	6	399964	5	NULL	NULL	0	NULL	second-order statistics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we construct a model for the acquired multiunit signal drawing on basic assumptions regarding the nature of a single neuron , which explains the second-order statistics of the raw electrode voltage measurements that are high-pass-filtered above 300 Hz .
	manualset3
93592	7	399964	5	NULL	NULL	0	NULL	raw electrode voltage measurements	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we construct a model for the acquired multiunit signal drawing on basic assumptions regarding the nature of a single neuron , which explains the second-order statistics of the raw electrode voltage measurements that are high-pass-filtered above 300 Hz .
	manualset3
93593	8	399964	5	NULL	NULL	0	NULL	300 Hz	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we construct a model for the acquired multiunit signal drawing on basic assumptions regarding the nature of a single neuron , which explains the second-order statistics of the raw electrode voltage measurements that are high-pass-filtered above 300 Hz .
	manualset3
93594	1	399965	5	NULL	NULL	0	NULL	up-regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we detected that the up-regulation of GCL and multi-drug resistance-associated protein ( MRP ) caused by As ( III ) was extremely low in H9c2 ( 2-1 ) cells compared with TRL1215 cells .
	manualset3
93595	2	399965	5	NULL	NULL	0	NULL	GCL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we detected that the up-regulation of GCL and multi-drug resistance-associated protein ( MRP ) caused by As ( III ) was extremely low in H9c2 ( 2-1 ) cells compared with TRL1215 cells .
	manualset3
93596	3	399965	5	NULL	NULL	0	NULL	multi-drug resistance-associated protein ( MRP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we detected that the up-regulation of GCL and multi-drug resistance-associated protein ( MRP ) caused by As ( III ) was extremely low in H9c2 ( 2-1 ) cells compared with TRL1215 cells .
	manualset3
93597	4	399965	5	NULL	NULL	0	NULL	As ( III )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we detected that the up-regulation of GCL and multi-drug resistance-associated protein ( MRP ) caused by As ( III ) was extremely low in H9c2 ( 2-1 ) cells compared with TRL1215 cells .
	manualset3
93598	5	399965	5	NULL	NULL	0	NULL	H9c2 ( 2-1 ) cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we detected that the up-regulation of GCL and multi-drug resistance-associated protein ( MRP ) caused by As ( III ) was extremely low in H9c2 ( 2-1 ) cells compared with TRL1215 cells .
	manualset3
93599	6	399965	5	NULL	NULL	0	NULL	TRL1215 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we detected that the up-regulation of GCL and multi-drug resistance-associated protein ( MRP ) caused by As ( III ) was extremely low in H9c2 ( 2-1 ) cells compared with TRL1215 cells .
	manualset3
93600	1	399966	5	NULL	NULL	0	NULL	association	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we did not find any association between the presence of IMCs and the lupus anticoagulant , IgG anticardiolipin antibodies , or extrarenal vascular manifestations .
	manualset3
93601	2	399966	5	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we did not find any association between the presence of IMCs and the lupus anticoagulant , IgG anticardiolipin antibodies , or extrarenal vascular manifestations .
	manualset3
93602	3	399966	5	NULL	NULL	0	NULL	IMCs	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we did not find any association between the presence of IMCs and the lupus anticoagulant , IgG anticardiolipin antibodies , or extrarenal vascular manifestations .
	manualset3
93603	4	399966	5	NULL	NULL	0	NULL	lupus anticoagulant	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we did not find any association between the presence of IMCs and the lupus anticoagulant , IgG anticardiolipin antibodies , or extrarenal vascular manifestations .
	manualset3
93604	5	399966	5	NULL	NULL	0	NULL	IgG anticardiolipin antibodies	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we did not find any association between the presence of IMCs and the lupus anticoagulant , IgG anticardiolipin antibodies , or extrarenal vascular manifestations .
	manualset3
93605	6	399966	5	NULL	NULL	0	NULL	extrarenal vascular manifestations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we did not find any association between the presence of IMCs and the lupus anticoagulant , IgG anticardiolipin antibodies , or extrarenal vascular manifestations .
	manualset3
93606	1	399967	5	NULL	NULL	0	NULL	delayed skin test	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Value of delayed skin test in elderly patients ) .
	manualset3
93607	2	399967	5	NULL	NULL	0	NULL	elderly patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Value of delayed skin test in elderly patients ) .
	manualset3
93608	1	399968	5	NULL	NULL	0	NULL	molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we discuss molecules of possible importance such as the glutathione-S-transferases , DNA repair genes , cyclin-dependent kinase inhibitor 2A , Brahma and connexins .
	manualset3
93609	2	399968	5	NULL	NULL	NULL	NULL	glutathione-S-transferases	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , we discuss molecules of possible importance such as the glutathione-S-transferases , DNA repair genes , cyclin-dependent kinase inhibitor 2A , Brahma and connexins .
	manualset3
93610	3	399968	5	NULL	NULL	0	NULL	DNA repair genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we discuss molecules of possible importance such as the glutathione-S-transferases , DNA repair genes , cyclin-dependent kinase inhibitor 2A , Brahma and connexins .
	manualset3
93611	4	399968	5	NULL	NULL	0	NULL	cyclin-dependent kinase inhibitor 2A 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we discuss molecules of possible importance such as the glutathione-S-transferases , DNA repair genes , cyclin-dependent kinase inhibitor 2A , Brahma and connexins .
	manualset3
93612	5	399968	5	NULL	NULL	0	NULL	Brahma	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we discuss molecules of possible importance such as the glutathione-S-transferases , DNA repair genes , cyclin-dependent kinase inhibitor 2A , Brahma and connexins .
	manualset3
93613	6	399968	5	NULL	NULL	0	NULL	connexins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we discuss molecules of possible importance such as the glutathione-S-transferases , DNA repair genes , cyclin-dependent kinase inhibitor 2A , Brahma and connexins .
	manualset3
93614	1	399969	5	NULL	NULL	0	NULL	activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we found both activation of ER stress response and autophagy in these patient fibroblasts .
	manualset3
93615	2	399969	5	NULL	NULL	0	NULL	ER stress response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we found both activation of ER stress response and autophagy in these patient fibroblasts .
	manualset3
93616	3	399969	5	NULL	NULL	0	NULL	autophagy	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we found both activation of ER stress response and autophagy in these patient fibroblasts .
	manualset3
93617	4	399969	5	NULL	NULL	0	NULL	patient fibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we found both activation of ER stress response and autophagy in these patient fibroblasts .
	manualset3
93618	1	399970	5	NULL	NULL	0	NULL	DW2282	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we found that DW2282 did not cause an increase in hemolysis in human blood .
	manualset3
93619	2	399970	5	NULL	NULL	0	NULL	hemolysis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we found that DW2282 did not cause an increase in hemolysis in human blood .
	manualset3
93620	3	399970	5	NULL	NULL	0	NULL	human blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we found that DW2282 did not cause an increase in hemolysis in human blood .
	manualset3
93621	1	399971	5	NULL	NULL	0	NULL	diabetic foot care service	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we have established a diabetic foot care service for outpatients , with the objective of preventing diabetes-related foot disease .
	manualset3
93622	2	399971	5	NULL	NULL	0	NULL	outpatients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we have established a diabetic foot care service for outpatients , with the objective of preventing diabetes-related foot disease .
	manualset3
93623	3	399971	5	NULL	NULL	0	NULL	diabetes-related foot disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we have established a diabetic foot care service for outpatients , with the objective of preventing diabetes-related foot disease .
	manualset3
93624	1	399972	5	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we present evidence that D ( 4 ) R activation tonically regulates the expression of AC1 in photoreceptors .
	manualset3
93625	2	399972	5	NULL	NULL	0	NULL	D ( 4 ) R activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we present evidence that D ( 4 ) R activation tonically regulates the expression of AC1 in photoreceptors .
	manualset3
93626	3	399972	5	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we present evidence that D ( 4 ) R activation tonically regulates the expression of AC1 in photoreceptors .
	manualset3
93627	4	399972	5	NULL	NULL	0	NULL	AC1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we present evidence that D ( 4 ) R activation tonically regulates the expression of AC1 in photoreceptors .
	manualset3
93628	5	399972	5	NULL	NULL	0	NULL	photoreceptors	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we present evidence that D ( 4 ) R activation tonically regulates the expression of AC1 in photoreceptors .
	manualset3
93629	1	399973	5	NULL	NULL	0	NULL	collagenase mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , whereas the collagenase mRNA was detected as early as 24 h posttreatment , the appearance of extracellular collagenase activity required 48 h. Using phalloidin to follow the organization of the cytoskeleton we observed that rTNF disrupted the parallel array of stress fibers normally observed in the perinuclear region .
	manualset3
93630	2	399973	5	NULL	NULL	0	NULL	24 h posttreatment	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , whereas the collagenase mRNA was detected as early as 24 h posttreatment , the appearance of extracellular collagenase activity required 48 h. Using phalloidin to follow the organization of the cytoskeleton we observed that rTNF disrupted the parallel array of stress fibers normally observed in the perinuclear region .
	manualset3
93631	3	399973	5	NULL	NULL	0	NULL	appearance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , whereas the collagenase mRNA was detected as early as 24 h posttreatment , the appearance of extracellular collagenase activity required 48 h. Using phalloidin to follow the organization of the cytoskeleton we observed that rTNF disrupted the parallel array of stress fibers normally observed in the perinuclear region .
	manualset3
93632	4	399973	5	NULL	NULL	0	NULL	extracellular collagenase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , whereas the collagenase mRNA was detected as early as 24 h posttreatment , the appearance of extracellular collagenase activity required 48 h. Using phalloidin to follow the organization of the cytoskeleton we observed that rTNF disrupted the parallel array of stress fibers normally observed in the perinuclear region .
	manualset3
93633	5	399973	5	NULL	NULL	0	NULL	48 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , whereas the collagenase mRNA was detected as early as 24 h posttreatment , the appearance of extracellular collagenase activity required 48 h. Using phalloidin to follow the organization of the cytoskeleton we observed that rTNF disrupted the parallel array of stress fibers normally observed in the perinuclear region .
	manualset3
93634	6	399973	5	NULL	NULL	0	NULL	phalloidin	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , whereas the collagenase mRNA was detected as early as 24 h posttreatment , the appearance of extracellular collagenase activity required 48 h. Using phalloidin to follow the organization of the cytoskeleton we observed that rTNF disrupted the parallel array of stress fibers normally observed in the perinuclear region .
	manualset3
93635	7	399973	5	NULL	NULL	0	NULL	organization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , whereas the collagenase mRNA was detected as early as 24 h posttreatment , the appearance of extracellular collagenase activity required 48 h. Using phalloidin to follow the organization of the cytoskeleton we observed that rTNF disrupted the parallel array of stress fibers normally observed in the perinuclear region .
	manualset3
93636	8	399973	5	NULL	NULL	0	NULL	cytoskeleton	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , whereas the collagenase mRNA was detected as early as 24 h posttreatment , the appearance of extracellular collagenase activity required 48 h. Using phalloidin to follow the organization of the cytoskeleton we observed that rTNF disrupted the parallel array of stress fibers normally observed in the perinuclear region .
	manualset3
93637	9	399973	5	NULL	NULL	0	NULL	rTNF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , whereas the collagenase mRNA was detected as early as 24 h posttreatment , the appearance of extracellular collagenase activity required 48 h. Using phalloidin to follow the organization of the cytoskeleton we observed that rTNF disrupted the parallel array of stress fibers normally observed in the perinuclear region .
	manualset3
93638	10	399973	5	NULL	NULL	0	NULL	parallel array	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , whereas the collagenase mRNA was detected as early as 24 h posttreatment , the appearance of extracellular collagenase activity required 48 h. Using phalloidin to follow the organization of the cytoskeleton we observed that rTNF disrupted the parallel array of stress fibers normally observed in the perinuclear region .
	manualset3
93639	11	399973	5	NULL	NULL	0	NULL	stress fibers	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , whereas the collagenase mRNA was detected as early as 24 h posttreatment , the appearance of extracellular collagenase activity required 48 h. Using phalloidin to follow the organization of the cytoskeleton we observed that rTNF disrupted the parallel array of stress fibers normally observed in the perinuclear region .
	manualset3
93640	12	399973	5	NULL	NULL	0	NULL	perinuclear region	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , whereas the collagenase mRNA was detected as early as 24 h posttreatment , the appearance of extracellular collagenase activity required 48 h. Using phalloidin to follow the organization of the cytoskeleton we observed that rTNF disrupted the parallel array of stress fibers normally observed in the perinuclear region .
	manualset3
93641	1	399974	5	NULL	NULL	0	NULL	histamine methyl transferase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , with regard to histamine methyl transferase activity , we were unable to demonstrate any difference in activity in the mucosal specimens obtained from the defined areas of the stomach .
	manualset3
93642	2	399974	5	NULL	NULL	0	NULL	difference in activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , with regard to histamine methyl transferase activity , we were unable to demonstrate any difference in activity in the mucosal specimens obtained from the defined areas of the stomach .
	manualset3
93643	3	399974	5	NULL	NULL	0	NULL	mucosal specimens	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , with regard to histamine methyl transferase activity , we were unable to demonstrate any difference in activity in the mucosal specimens obtained from the defined areas of the stomach .
	manualset3
93644	4	399974	5	NULL	NULL	0	NULL	defined areas of the stomach	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , with regard to histamine methyl transferase activity , we were unable to demonstrate any difference in activity in the mucosal specimens obtained from the defined areas of the stomach .
	manualset3
93645	1	399975	5	NULL	NULL	0	NULL	multidetector computed tomography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Value of multidetector computed tomography and digital subtraction angiography in assessment of arterio-venous fistula for hemodialysis -- own experiences ) .
	manualset3
93646	2	399975	5	NULL	NULL	0	NULL	digital subtraction angiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Value of multidetector computed tomography and digital subtraction angiography in assessment of arterio-venous fistula for hemodialysis -- own experiences ) .
	manualset3
93647	3	399975	5	NULL	NULL	0	NULL	assessment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Value of multidetector computed tomography and digital subtraction angiography in assessment of arterio-venous fistula for hemodialysis -- own experiences ) .
	manualset3
93648	4	399975	5	NULL	NULL	0	NULL	arterio-venous fistula	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Value of multidetector computed tomography and digital subtraction angiography in assessment of arterio-venous fistula for hemodialysis -- own experiences ) .
	manualset3
93649	5	399975	5	NULL	NULL	0	NULL	hemodialysis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Value of multidetector computed tomography and digital subtraction angiography in assessment of arterio-venous fistula for hemodialysis -- own experiences ) .
	manualset3
93650	6	399975	5	NULL	NULL	0	NULL	own experiences	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Value of multidetector computed tomography and digital subtraction angiography in assessment of arterio-venous fistula for hemodialysis -- own experiences ) .
	manualset3
93651	1	399976	5	NULL	NULL	0	NULL	IL-6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to IL-6 , the IL-6 cytokine family includes IL-11 , ciliary neurotrophic factor ( cntf ) , cardiotrophin-1 ( CT-1 ) , cardiotrophin-like cytokine ( CLC ) , leukemia inhibitory factor ( LIF ) y Oncostatin M ( OsM ) .
	manualset3
93652	2	399976	5	NULL	NULL	0	NULL	IL-6 cytokine family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to IL-6 , the IL-6 cytokine family includes IL-11 , ciliary neurotrophic factor ( cntf ) , cardiotrophin-1 ( CT-1 ) , cardiotrophin-like cytokine ( CLC ) , leukemia inhibitory factor ( LIF ) y Oncostatin M ( OsM ) .
	manualset3
93653	3	399976	5	NULL	NULL	0	NULL	IL-11	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to IL-6 , the IL-6 cytokine family includes IL-11 , ciliary neurotrophic factor ( cntf ) , cardiotrophin-1 ( CT-1 ) , cardiotrophin-like cytokine ( CLC ) , leukemia inhibitory factor ( LIF ) y Oncostatin M ( OsM ) .
	manualset3
93654	4	399976	5	NULL	NULL	0	NULL	ciliary neurotrophic factor ( cntf )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to IL-6 , the IL-6 cytokine family includes IL-11 , ciliary neurotrophic factor ( cntf ) , cardiotrophin-1 ( CT-1 ) , cardiotrophin-like cytokine ( CLC ) , leukemia inhibitory factor ( LIF ) y Oncostatin M ( OsM ) .
	manualset3
93655	5	399976	5	NULL	NULL	0	NULL	cardiotrophin-1 ( CT-1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to IL-6 , the IL-6 cytokine family includes IL-11 , ciliary neurotrophic factor ( cntf ) , cardiotrophin-1 ( CT-1 ) , cardiotrophin-like cytokine ( CLC ) , leukemia inhibitory factor ( LIF ) y Oncostatin M ( OsM ) .
	manualset3
93656	6	399976	5	NULL	NULL	0	NULL	cardiotrophin-like cytokine ( CLC )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to IL-6 , the IL-6 cytokine family includes IL-11 , ciliary neurotrophic factor ( cntf ) , cardiotrophin-1 ( CT-1 ) , cardiotrophin-like cytokine ( CLC ) , leukemia inhibitory factor ( LIF ) y Oncostatin M ( OsM ) .
	manualset3
93657	7	399976	5	NULL	NULL	0	NULL	leukemia inhibitory factor ( LIF )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to IL-6 , the IL-6 cytokine family includes IL-11 , ciliary neurotrophic factor ( cntf ) , cardiotrophin-1 ( CT-1 ) , cardiotrophin-like cytokine ( CLC ) , leukemia inhibitory factor ( LIF ) y Oncostatin M ( OsM ) .
	manualset3
93658	8	399976	5	NULL	NULL	0	NULL	Oncostatin M ( OsM )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to IL-6 , the IL-6 cytokine family includes IL-11 , ciliary neurotrophic factor ( cntf ) , cardiotrophin-1 ( CT-1 ) , cardiotrophin-like cytokine ( CLC ) , leukemia inhibitory factor ( LIF ) y Oncostatin M ( OsM ) .
	manualset3
93659	1	399977	5	NULL	NULL	0	NULL	TBI	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to TBI , 19 dogs were given anti-class II monoclonal antibody ( mAb ) 7.2 , either alone or combined with a second anti-class II mAb , HB10a , at doses of 0.2 or 0.4 mg/kg/day on days -5 to 0 or -1 to +3 .
	manualset3
93660	2	399977	5	NULL	NULL	0	NULL	19 dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to TBI , 19 dogs were given anti-class II monoclonal antibody ( mAb ) 7.2 , either alone or combined with a second anti-class II mAb , HB10a , at doses of 0.2 or 0.4 mg/kg/day on days -5 to 0 or -1 to +3 .
	manualset3
93661	3	399977	5	NULL	NULL	0	NULL	anti-class II monoclonal antibody ( mAb ) 7.2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to TBI , 19 dogs were given anti-class II monoclonal antibody ( mAb ) 7.2 , either alone or combined with a second anti-class II mAb , HB10a , at doses of 0.2 or 0.4 mg/kg/day on days -5 to 0 or -1 to +3 .
	manualset3
93662	4	399977	5	NULL	NULL	0	NULL	anti-class II mAb , HB10a	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to TBI , 19 dogs were given anti-class II monoclonal antibody ( mAb ) 7.2 , either alone or combined with a second anti-class II mAb , HB10a , at doses of 0.2 or 0.4 mg/kg/day on days -5 to 0 or -1 to +3 .
	manualset3
93663	5	399977	5	NULL	NULL	0	NULL	doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to TBI , 19 dogs were given anti-class II monoclonal antibody ( mAb ) 7.2 , either alone or combined with a second anti-class II mAb , HB10a , at doses of 0.2 or 0.4 mg/kg/day on days -5 to 0 or -1 to +3 .
	manualset3
93664	6	399977	5	NULL	NULL	0	NULL	0.2 or 0.4 mg/kg/day	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to TBI , 19 dogs were given anti-class II monoclonal antibody ( mAb ) 7.2 , either alone or combined with a second anti-class II mAb , HB10a , at doses of 0.2 or 0.4 mg/kg/day on days -5 to 0 or -1 to +3 .
	manualset3
93665	7	399977	5	NULL	NULL	0	NULL	days -5 to 0	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to TBI , 19 dogs were given anti-class II monoclonal antibody ( mAb ) 7.2 , either alone or combined with a second anti-class II mAb , HB10a , at doses of 0.2 or 0.4 mg/kg/day on days -5 to 0 or -1 to +3 .
	manualset3
93666	8	399977	5	NULL	NULL	0	NULL	days -1 to +3	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to TBI , 19 dogs were given anti-class II monoclonal antibody ( mAb ) 7.2 , either alone or combined with a second anti-class II mAb , HB10a , at doses of 0.2 or 0.4 mg/kg/day on days -5 to 0 or -1 to +3 .
	manualset3
93667	1	399978	5	NULL	NULL	0	NULL	testosterone precursors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to being testosterone precursors in vivo , either may impart its own transcriptional regulation of AR .
	manualset3
93668	2	399978	5	NULL	NULL	0	NULL	transcriptional regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to being testosterone precursors in vivo , either may impart its own transcriptional regulation of AR .
	manualset3
93669	3	399978	5	NULL	NULL	0	NULL	AR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to being testosterone precursors in vivo , either may impart its own transcriptional regulation of AR .
	manualset3
93670	1	399979	5	NULL	NULL	0	NULL	duplex Doppler ultrasound	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to duplex Doppler ultrasound , using a gold standard test of vertebral artery testing by way of magnetic resonance angiography ( MRA ) would further improve data on the diagnostic utility of the CPTQ .
	manualset3
93671	2	399979	5	NULL	NULL	NULL	NULL	gold standard test	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition to duplex Doppler ultrasound , using a gold standard test of vertebral artery testing by way of magnetic resonance angiography ( MRA ) would further improve data on the diagnostic utility of the CPTQ .
	manualset3
93672	3	399979	5	NULL	NULL	0	NULL	vertebral artery testing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to duplex Doppler ultrasound , using a gold standard test of vertebral artery testing by way of magnetic resonance angiography ( MRA ) would further improve data on the diagnostic utility of the CPTQ .
	manualset3
93673	4	399979	5	NULL	NULL	0	NULL	magnetic resonance angiography ( MRA )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to duplex Doppler ultrasound , using a gold standard test of vertebral artery testing by way of magnetic resonance angiography ( MRA ) would further improve data on the diagnostic utility of the CPTQ .
	manualset3
93674	5	399979	5	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to duplex Doppler ultrasound , using a gold standard test of vertebral artery testing by way of magnetic resonance angiography ( MRA ) would further improve data on the diagnostic utility of the CPTQ .
	manualset3
93675	6	399979	5	NULL	NULL	NULL	NULL	CPTQ	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition to duplex Doppler ultrasound , using a gold standard test of vertebral artery testing by way of magnetic resonance angiography ( MRA ) would further improve data on the diagnostic utility of the CPTQ .
	manualset3
98566	7	399979	5	NULL	NULL	0	NULL	diagnostic utility	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to duplex Doppler ultrasound , using a gold standard test of vertebral artery testing by way of magnetic resonance angiography ( MRA ) would further improve data on the diagnostic utility of the CPTQ .
	manualset3
93676	1	399980	5	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to effects in cells directly targeted with heavy ions , there is mounting evidence for nontargeted biological effects in cells that have not themselves been directly irradiated .
	manualset3
93677	2	399980	5	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to effects in cells directly targeted with heavy ions , there is mounting evidence for nontargeted biological effects in cells that have not themselves been directly irradiated .
	manualset3
93678	3	399980	5	NULL	NULL	0	NULL	heavy ions 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to effects in cells directly targeted with heavy ions , there is mounting evidence for nontargeted biological effects in cells that have not themselves been directly irradiated .
	manualset3
93679	4	399980	5	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to effects in cells directly targeted with heavy ions , there is mounting evidence for nontargeted biological effects in cells that have not themselves been directly irradiated .
	manualset3
93680	5	399980	5	NULL	NULL	0	NULL	nontargeted biological effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to effects in cells directly targeted with heavy ions , there is mounting evidence for nontargeted biological effects in cells that have not themselves been directly irradiated .
	manualset3
93681	6	399980	5	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to effects in cells directly targeted with heavy ions , there is mounting evidence for nontargeted biological effects in cells that have not themselves been directly irradiated .
	manualset3
93682	1	399981	5	NULL	NULL	0	NULL	etiologic assessment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to etiologic assessment using clinical and laboratory methods and echocardiography , the patients ' drinking habits were evaluated by recording the amount of alcohol used during the week preceding AF , by responses to the CAGE ( Cut , Annoying , Guilt , Eye ; see below ) questionnaire ( a screening test for alcohol abuse ) and by selected laboratory tests .
	manualset3
93683	2	399981	5	NULL	NULL	0	NULL	clinical and laboratory methods	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to etiologic assessment using clinical and laboratory methods and echocardiography , the patients ' drinking habits were evaluated by recording the amount of alcohol used during the week preceding AF , by responses to the CAGE ( Cut , Annoying , Guilt , Eye ; see below ) questionnaire ( a screening test for alcohol abuse ) and by selected laboratory tests .
	manualset3
93684	3	399981	5	NULL	NULL	0	NULL	echocardiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to etiologic assessment using clinical and laboratory methods and echocardiography , the patients ' drinking habits were evaluated by recording the amount of alcohol used during the week preceding AF , by responses to the CAGE ( Cut , Annoying , Guilt , Eye ; see below ) questionnaire ( a screening test for alcohol abuse ) and by selected laboratory tests .
	manualset3
93685	4	399981	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to etiologic assessment using clinical and laboratory methods and echocardiography , the patients ' drinking habits were evaluated by recording the amount of alcohol used during the week preceding AF , by responses to the CAGE ( Cut , Annoying , Guilt , Eye ; see below ) questionnaire ( a screening test for alcohol abuse ) and by selected laboratory tests .
	manualset3
93686	5	399981	5	NULL	NULL	0	NULL	drinking habits	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to etiologic assessment using clinical and laboratory methods and echocardiography , the patients ' drinking habits were evaluated by recording the amount of alcohol used during the week preceding AF , by responses to the CAGE ( Cut , Annoying , Guilt , Eye ; see below ) questionnaire ( a screening test for alcohol abuse ) and by selected laboratory tests .
	manualset3
93687	6	399981	5	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to etiologic assessment using clinical and laboratory methods and echocardiography , the patients ' drinking habits were evaluated by recording the amount of alcohol used during the week preceding AF , by responses to the CAGE ( Cut , Annoying , Guilt , Eye ; see below ) questionnaire ( a screening test for alcohol abuse ) and by selected laboratory tests .
	manualset3
93688	7	399981	5	NULL	NULL	0	NULL	alcohol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to etiologic assessment using clinical and laboratory methods and echocardiography , the patients ' drinking habits were evaluated by recording the amount of alcohol used during the week preceding AF , by responses to the CAGE ( Cut , Annoying , Guilt , Eye ; see below ) questionnaire ( a screening test for alcohol abuse ) and by selected laboratory tests .
	manualset3
93689	8	399981	5	NULL	NULL	0	NULL	week	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to etiologic assessment using clinical and laboratory methods and echocardiography , the patients ' drinking habits were evaluated by recording the amount of alcohol used during the week preceding AF , by responses to the CAGE ( Cut , Annoying , Guilt , Eye ; see below ) questionnaire ( a screening test for alcohol abuse ) and by selected laboratory tests .
	manualset3
93690	9	399981	5	NULL	NULL	0	NULL	AF	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to etiologic assessment using clinical and laboratory methods and echocardiography , the patients ' drinking habits were evaluated by recording the amount of alcohol used during the week preceding AF , by responses to the CAGE ( Cut , Annoying , Guilt , Eye ; see below ) questionnaire ( a screening test for alcohol abuse ) and by selected laboratory tests .
	manualset3
93691	10	399981	5	NULL	NULL	0	NULL	CAGE ( Cut , Annoying , Guilt , Eye ; see below ) questionnaire	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to etiologic assessment using clinical and laboratory methods and echocardiography , the patients ' drinking habits were evaluated by recording the amount of alcohol used during the week preceding AF , by responses to the CAGE ( Cut , Annoying , Guilt , Eye ; see below ) questionnaire ( a screening test for alcohol abuse ) and by selected laboratory tests .
	manualset3
93692	11	399981	5	NULL	NULL	0	NULL	screening test	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to etiologic assessment using clinical and laboratory methods and echocardiography , the patients ' drinking habits were evaluated by recording the amount of alcohol used during the week preceding AF , by responses to the CAGE ( Cut , Annoying , Guilt , Eye ; see below ) questionnaire ( a screening test for alcohol abuse ) and by selected laboratory tests .
	manualset3
93693	12	399981	5	NULL	NULL	0	NULL	alcohol abuse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to etiologic assessment using clinical and laboratory methods and echocardiography , the patients ' drinking habits were evaluated by recording the amount of alcohol used during the week preceding AF , by responses to the CAGE ( Cut , Annoying , Guilt , Eye ; see below ) questionnaire ( a screening test for alcohol abuse ) and by selected laboratory tests .
	manualset3
93694	13	399981	5	NULL	NULL	0	NULL	selected laboratory tests	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to etiologic assessment using clinical and laboratory methods and echocardiography , the patients ' drinking habits were evaluated by recording the amount of alcohol used during the week preceding AF , by responses to the CAGE ( Cut , Annoying , Guilt , Eye ; see below ) questionnaire ( a screening test for alcohol abuse ) and by selected laboratory tests .
	manualset3
93855	1	399982	5	NULL	NULL	NULL	NULL	sugar	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition to extensive contacts with the sugar , O-GlcNAcase recognizes the peptide backbone through hydrophobic interactions and intramolecular hydrogen bonds , while avoiding interactions with the glycopeptide side chains .
	manualset3
93856	2	399982	5	NULL	NULL	0	NULL	O-GlcNAcase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to extensive contacts with the sugar , O-GlcNAcase recognizes the peptide backbone through hydrophobic interactions and intramolecular hydrogen bonds , while avoiding interactions with the glycopeptide side chains .
	manualset3
93857	3	399982	5	NULL	NULL	0	NULL	peptide backbone	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to extensive contacts with the sugar , O-GlcNAcase recognizes the peptide backbone through hydrophobic interactions and intramolecular hydrogen bonds , while avoiding interactions with the glycopeptide side chains .
	manualset3
93858	4	399982	5	NULL	NULL	0	NULL	hydrophobic interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to extensive contacts with the sugar , O-GlcNAcase recognizes the peptide backbone through hydrophobic interactions and intramolecular hydrogen bonds , while avoiding interactions with the glycopeptide side chains .
	manualset3
93859	5	399982	5	NULL	NULL	NULL	NULL	intramolecular hydrogen bonds	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition to extensive contacts with the sugar , O-GlcNAcase recognizes the peptide backbone through hydrophobic interactions and intramolecular hydrogen bonds , while avoiding interactions with the glycopeptide side chains .
	manualset3
93860	6	399982	5	NULL	NULL	0	NULL	interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to extensive contacts with the sugar , O-GlcNAcase recognizes the peptide backbone through hydrophobic interactions and intramolecular hydrogen bonds , while avoiding interactions with the glycopeptide side chains .
	manualset3
93861	7	399982	5	NULL	NULL	0	NULL	glycopeptide side chains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to extensive contacts with the sugar , O-GlcNAcase recognizes the peptide backbone through hydrophobic interactions and intramolecular hydrogen bonds , while avoiding interactions with the glycopeptide side chains .
	manualset3
93998	8	399982	5	NULL	NULL	0	NULL	extensive contacts	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to extensive contacts with the sugar , O-GlcNAcase recognizes the peptide backbone through hydrophobic interactions and intramolecular hydrogen bonds , while avoiding interactions with the glycopeptide side chains .
	manualset3
93862	1	399983	5	NULL	NULL	0	NULL	skills	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to increasing skills in the health outcomes management arena , nurses will benefit from a continual increase in knowledge of case management , clinical pathways , and guidelines .
	manualset3
93863	2	399983	5	NULL	NULL	NULL	NULL	health outcomes management arena	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition to increasing skills in the health outcomes management arena , nurses will benefit from a continual increase in knowledge of case management , clinical pathways , and guidelines .
	manualset3
93864	3	399983	5	NULL	NULL	0	NULL	nurses	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to increasing skills in the health outcomes management arena , nurses will benefit from a continual increase in knowledge of case management , clinical pathways , and guidelines .
	manualset3
93865	4	399983	5	NULL	NULL	0	NULL	knowledge	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to increasing skills in the health outcomes management arena , nurses will benefit from a continual increase in knowledge of case management , clinical pathways , and guidelines .
	manualset3
93866	5	399983	5	NULL	NULL	NULL	NULL	case management	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition to increasing skills in the health outcomes management arena , nurses will benefit from a continual increase in knowledge of case management , clinical pathways , and guidelines .
	manualset3
93867	6	399983	5	NULL	NULL	NULL	NULL	clinical pathways	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition to increasing skills in the health outcomes management arena , nurses will benefit from a continual increase in knowledge of case management , clinical pathways , and guidelines .
	manualset3
93868	7	399983	5	NULL	NULL	0	NULL	guidelines	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to increasing skills in the health outcomes management arena , nurses will benefit from a continual increase in knowledge of case management , clinical pathways , and guidelines .
	manualset3
93869	1	399984	5	NULL	NULL	0	NULL	nuclear magnetic resonance tomography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Value of nuclear magnetic resonance tomography in diagnosis of infrarenal abdominal aortic aneurysms .
	manualset3
93870	2	399984	5	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Value of nuclear magnetic resonance tomography in diagnosis of infrarenal abdominal aortic aneurysms .
	manualset3
93871	3	399984	5	NULL	NULL	0	NULL	infrarenal abdominal aortic aneurysms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Value of nuclear magnetic resonance tomography in diagnosis of infrarenal abdominal aortic aneurysms .
	manualset3
93872	1	399985	5	NULL	NULL	0	NULL	angiogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to mediating angiogenesis and endothelial cell growth , VPF has been reported to be a potent mediator of increased microvascular permeability in vivo .
	manualset3
93873	2	399985	5	NULL	NULL	0	NULL	endothelial cell growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to mediating angiogenesis and endothelial cell growth , VPF has been reported to be a potent mediator of increased microvascular permeability in vivo .
	manualset3
93874	3	399985	5	NULL	NULL	0	NULL	VPF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to mediating angiogenesis and endothelial cell growth , VPF has been reported to be a potent mediator of increased microvascular permeability in vivo .
	manualset3
93875	4	399985	5	NULL	NULL	0	NULL	 potent mediator	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to mediating angiogenesis and endothelial cell growth , VPF has been reported to be a potent mediator of increased microvascular permeability in vivo .
	manualset3
93876	5	399985	5	NULL	NULL	NULL	NULL	microvascular permeability	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition to mediating angiogenesis and endothelial cell growth , VPF has been reported to be a potent mediator of increased microvascular permeability in vivo .
	manualset3
93877	1	399986	5	NULL	NULL	0	NULL	knowledge	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to our previous knowledge that Calu-3 cells express KCNQ1 , using reverse transcriptase polymerase chain reaction we determined expression of KCNQ3 , KCNQ4 and KCNQ5 mRNA transcripts .
	manualset3
93878	2	399986	5	NULL	NULL	0	NULL	Calu-3 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to our previous knowledge that Calu-3 cells express KCNQ1 , using reverse transcriptase polymerase chain reaction we determined expression of KCNQ3 , KCNQ4 and KCNQ5 mRNA transcripts .
	manualset3
93879	3	399986	5	NULL	NULL	0	NULL	KCNQ1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to our previous knowledge that Calu-3 cells express KCNQ1 , using reverse transcriptase polymerase chain reaction we determined expression of KCNQ3 , KCNQ4 and KCNQ5 mRNA transcripts .
	manualset3
93880	4	399986	5	NULL	NULL	0	NULL	reverse transcriptase polymerase chain reaction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to our previous knowledge that Calu-3 cells express KCNQ1 , using reverse transcriptase polymerase chain reaction we determined expression of KCNQ3 , KCNQ4 and KCNQ5 mRNA transcripts .
	manualset3
93881	5	399986	5	NULL	NULL	0	NULL	expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to our previous knowledge that Calu-3 cells express KCNQ1 , using reverse transcriptase polymerase chain reaction we determined expression of KCNQ3 , KCNQ4 and KCNQ5 mRNA transcripts .
	manualset3
93882	6	399986	5	NULL	NULL	0	NULL	KCNQ3 mRNA transcripts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to our previous knowledge that Calu-3 cells express KCNQ1 , using reverse transcriptase polymerase chain reaction we determined expression of KCNQ3 , KCNQ4 and KCNQ5 mRNA transcripts .
	manualset3
93883	7	399986	5	NULL	NULL	NULL	NULL	KCNQ4 mRNA transcripts	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition to our previous knowledge that Calu-3 cells express KCNQ1 , using reverse transcriptase polymerase chain reaction we determined expression of KCNQ3 , KCNQ4 and KCNQ5 mRNA transcripts .
	manualset3
93884	8	399986	5	NULL	NULL	0	NULL	KCNQ5 mRNA transcripts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to our previous knowledge that Calu-3 cells express KCNQ1 , using reverse transcriptase polymerase chain reaction we determined expression of KCNQ3 , KCNQ4 and KCNQ5 mRNA transcripts .
	manualset3
93885	1	399987	5	NULL	NULL	0	NULL	pharmacologic therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to pharmacologic therapy , patient education , cognitive behavioral therapy , aerobic exercise , and strength and flexibility training are important components of care .
	manualset3
93886	2	399987	5	NULL	NULL	0	NULL	patient education	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to pharmacologic therapy , patient education , cognitive behavioral therapy , aerobic exercise , and strength and flexibility training are important components of care .
	manualset3
93887	3	399987	5	NULL	NULL	0	NULL	cognitive behavioral therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to pharmacologic therapy , patient education , cognitive behavioral therapy , aerobic exercise , and strength and flexibility training are important components of care .
	manualset3
93888	4	399987	5	NULL	NULL	0	NULL	aerobic exercise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to pharmacologic therapy , patient education , cognitive behavioral therapy , aerobic exercise , and strength and flexibility training are important components of care .
	manualset3
93889	5	399987	5	NULL	NULL	0	NULL	strength and flexibility training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to pharmacologic therapy , patient education , cognitive behavioral therapy , aerobic exercise , and strength and flexibility training are important components of care .
	manualset3
93890	6	399987	5	NULL	NULL	0	NULL	components	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to pharmacologic therapy , patient education , cognitive behavioral therapy , aerobic exercise , and strength and flexibility training are important components of care .
	manualset3
93891	7	399987	5	NULL	NULL	0	NULL	care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to pharmacologic therapy , patient education , cognitive behavioral therapy , aerobic exercise , and strength and flexibility training are important components of care .
	manualset3
93892	1	399988	5	NULL	NULL	0	NULL	 polypurine-polypyrimidine sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to polypurine-polypyrimidine sequences .
	manualset3
93893	1	399989	5	NULL	NULL	0	NULL	effective symptom relief	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to providing effective symptom relief in malignant carcinoid syndrome , octreotide can also be used for diagnostic purposes .
	manualset3
93894	2	399989	5	NULL	NULL	0	NULL	malignant carcinoid syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to providing effective symptom relief in malignant carcinoid syndrome , octreotide can also be used for diagnostic purposes .
	manualset3
93895	3	399989	5	NULL	NULL	0	NULL	octreotide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to providing effective symptom relief in malignant carcinoid syndrome , octreotide can also be used for diagnostic purposes .
	manualset3
93896	4	399989	5	NULL	NULL	0	NULL	diagnostic purposes	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to providing effective symptom relief in malignant carcinoid syndrome , octreotide can also be used for diagnostic purposes .
	manualset3
93897	1	399990	5	NULL	NULL	0	NULL	efficient and accurate records	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to providing efficient and accurate records for individual patients , large databases of EHRs contain valuable information about overall patient populations .
	manualset3
93898	2	399990	5	NULL	NULL	0	NULL	individual patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to providing efficient and accurate records for individual patients , large databases of EHRs contain valuable information about overall patient populations .
	manualset3
93899	3	399990	5	NULL	NULL	0	NULL	large databases	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to providing efficient and accurate records for individual patients , large databases of EHRs contain valuable information about overall patient populations .
	manualset3
93900	4	399990	5	NULL	NULL	0	NULL	EHRs	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to providing efficient and accurate records for individual patients , large databases of EHRs contain valuable information about overall patient populations .
	manualset3
93901	5	399990	5	NULL	NULL	0	NULL	valuable information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to providing efficient and accurate records for individual patients , large databases of EHRs contain valuable information about overall patient populations .
	manualset3
93902	6	399990	5	NULL	NULL	0	NULL	overall patient populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to providing efficient and accurate records for individual patients , large databases of EHRs contain valuable information about overall patient populations .
	manualset3
93903	1	399991	5	NULL	NULL	0	NULL	substantial amounts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to substantial amounts of unchanged drug , three radiolabelled metabolites ( two major and one minor ) were detected in the urine during the 6 hour collection period following the administration of ( 1-14C ) - and ( 2 ' -14 C ) - streptozotocin .
	manualset3
93904	2	399991	5	NULL	NULL	0	NULL	unchanged drug	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to substantial amounts of unchanged drug , three radiolabelled metabolites ( two major and one minor ) were detected in the urine during the 6 hour collection period following the administration of ( 1-14C ) - and ( 2 ' -14 C ) - streptozotocin .
	manualset3
93905	3	399991	5	NULL	NULL	0	NULL	three radiolabelled metabolites	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to substantial amounts of unchanged drug , three radiolabelled metabolites ( two major and one minor ) were detected in the urine during the 6 hour collection period following the administration of ( 1-14C ) - and ( 2 ' -14 C ) - streptozotocin .
	manualset3
93906	4	399991	5	NULL	NULL	0	NULL	urine													NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to substantial amounts of unchanged drug , three radiolabelled metabolites ( two major and one minor ) were detected in the urine during the 6 hour collection period following the administration of ( 1-14C ) - and ( 2 ' -14 C ) - streptozotocin .
	manualset3
93907	5	399991	5	NULL	NULL	0	NULL	6 hour collection period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to substantial amounts of unchanged drug , three radiolabelled metabolites ( two major and one minor ) were detected in the urine during the 6 hour collection period following the administration of ( 1-14C ) - and ( 2 ' -14 C ) - streptozotocin .
	manualset3
93908	6	399991	5	NULL	NULL	0	NULL	administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to substantial amounts of unchanged drug , three radiolabelled metabolites ( two major and one minor ) were detected in the urine during the 6 hour collection period following the administration of ( 1-14C ) - and ( 2 ' -14 C ) - streptozotocin .
	manualset3
93909	7	399991	5	NULL	NULL	0	NULL	( 1-14C ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to substantial amounts of unchanged drug , three radiolabelled metabolites ( two major and one minor ) were detected in the urine during the 6 hour collection period following the administration of ( 1-14C ) - and ( 2 ' -14 C ) - streptozotocin .
	manualset3
93910	8	399991	5	NULL	NULL	0	NULL	 ( 2 ' -14 C )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to substantial amounts of unchanged drug , three radiolabelled metabolites ( two major and one minor ) were detected in the urine during the 6 hour collection period following the administration of ( 1-14C ) - and ( 2 ' -14 C ) - streptozotocin .
	manualset3
93911	9	399991	5	NULL	NULL	0	NULL	streptozotocin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to substantial amounts of unchanged drug , three radiolabelled metabolites ( two major and one minor ) were detected in the urine during the 6 hour collection period following the administration of ( 1-14C ) - and ( 2 ' -14 C ) - streptozotocin .
	manualset3
93912	1	399992	5	NULL	NULL	NULL	NULL	alterations	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition to the alterations at the mRNA level , changes also can occur at the DNA level in the EGF system .
	manualset3
93913	2	399992	5	NULL	NULL	0	NULL	mRNA level 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the alterations at the mRNA level , changes also can occur at the DNA level in the EGF system .
	manualset3
93914	3	399992	5	NULL	NULL	0	NULL	DNA level	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the alterations at the mRNA level , changes also can occur at the DNA level in the EGF system .
	manualset3
93915	4	399992	5	NULL	NULL	0	NULL	EGF system	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the alterations at the mRNA level , changes also can occur at the DNA level in the EGF system .
	manualset3
93916	1	399993	5	NULL	NULL	0	NULL	clinical data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Value of some clinical and radiological data in determining the frequency of infiltration of gastric cancer into the pancreas and their mathematical analysis ) .
	manualset3
93917	2	399993	5	NULL	NULL	0	NULL	radiological data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Value of some clinical and radiological data in determining the frequency of infiltration of gastric cancer into the pancreas and their mathematical analysis ) .
	manualset3
93918	3	399993	5	NULL	NULL	0	NULL	frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Value of some clinical and radiological data in determining the frequency of infiltration of gastric cancer into the pancreas and their mathematical analysis ) .
	manualset3
93919	4	399993	5	NULL	NULL	0	NULL	infiltration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Value of some clinical and radiological data in determining the frequency of infiltration of gastric cancer into the pancreas and their mathematical analysis ) .
	manualset3
93920	5	399993	5	NULL	NULL	0	NULL	gastric cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Value of some clinical and radiological data in determining the frequency of infiltration of gastric cancer into the pancreas and their mathematical analysis ) .
	manualset3
93921	6	399993	5	NULL	NULL	0	NULL	pancreas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Value of some clinical and radiological data in determining the frequency of infiltration of gastric cancer into the pancreas and their mathematical analysis ) .
	manualset3
93922	7	399993	5	NULL	NULL	0	NULL	mathematical analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Value of some clinical and radiological data in determining the frequency of infiltration of gastric cancer into the pancreas and their mathematical analysis ) .
	manualset3
93923	1	399994	5	NULL	NULL	0	NULL	drug treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the drug treatment , the opportunity for social interaction with either a sober or intoxicated conspecific was varied across groups ( N = 8 rats/group ) .
	manualset3
93924	2	399994	5	NULL	NULL	0	NULL	opportunity	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the drug treatment , the opportunity for social interaction with either a sober or intoxicated conspecific was varied across groups ( N = 8 rats/group ) .
	manualset3
93925	3	399994	5	NULL	NULL	0	NULL	social interaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the drug treatment , the opportunity for social interaction with either a sober or intoxicated conspecific was varied across groups ( N = 8 rats/group ) .
	manualset3
93926	4	399994	5	NULL	NULL	0	NULL	sober or intoxicated conspecific	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the drug treatment , the opportunity for social interaction with either a sober or intoxicated conspecific was varied across groups ( N = 8 rats/group ) .
	manualset3
93927	5	399994	5	NULL	NULL	0	NULL	groups	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the drug treatment , the opportunity for social interaction with either a sober or intoxicated conspecific was varied across groups ( N = 8 rats/group ) .
	manualset3
93928	6	399994	5	NULL	NULL	0	NULL	( N = 8 rats/group )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the drug treatment , the opportunity for social interaction with either a sober or intoxicated conspecific was varied across groups ( N = 8 rats/group ) .
	manualset3
93929	1	399995	5	NULL	NULL	0	NULL	common mental health issues	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the need to address common mental health issues such as depression , given that sleep problems are modifiable and potentially less stigmatizing than mental health problems , assessing and addressing insomnia and nightmares in survivors of interpersonal violence warrants strong clinical consideration and further investigation .
	manualset3
93930	2	399995	5	NULL	NULL	0	NULL	depression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the need to address common mental health issues such as depression , given that sleep problems are modifiable and potentially less stigmatizing than mental health problems , assessing and addressing insomnia and nightmares in survivors of interpersonal violence warrants strong clinical consideration and further investigation .
	manualset3
93931	3	399995	5	NULL	NULL	0	NULL	sleep problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the need to address common mental health issues such as depression , given that sleep problems are modifiable and potentially less stigmatizing than mental health problems , assessing and addressing insomnia and nightmares in survivors of interpersonal violence warrants strong clinical consideration and further investigation .
	manualset3
93932	4	399995	5	NULL	NULL	0	NULL	mental health problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the need to address common mental health issues such as depression , given that sleep problems are modifiable and potentially less stigmatizing than mental health problems , assessing and addressing insomnia and nightmares in survivors of interpersonal violence warrants strong clinical consideration and further investigation .
	manualset3
93933	5	399995	5	NULL	NULL	0	NULL	insomnia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the need to address common mental health issues such as depression , given that sleep problems are modifiable and potentially less stigmatizing than mental health problems , assessing and addressing insomnia and nightmares in survivors of interpersonal violence warrants strong clinical consideration and further investigation .
	manualset3
93934	6	399995	5	NULL	NULL	NULL	NULL	nightmares	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition to the need to address common mental health issues such as depression , given that sleep problems are modifiable and potentially less stigmatizing than mental health problems , assessing and addressing insomnia and nightmares in survivors of interpersonal violence warrants strong clinical consideration and further investigation .
	manualset3
93935	7	399995	5	NULL	NULL	0	NULL	survivors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the need to address common mental health issues such as depression , given that sleep problems are modifiable and potentially less stigmatizing than mental health problems , assessing and addressing insomnia and nightmares in survivors of interpersonal violence warrants strong clinical consideration and further investigation .
	manualset3
93936	8	399995	5	NULL	NULL	0	NULL	interpersonal violence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the need to address common mental health issues such as depression , given that sleep problems are modifiable and potentially less stigmatizing than mental health problems , assessing and addressing insomnia and nightmares in survivors of interpersonal violence warrants strong clinical consideration and further investigation .
	manualset3
93937	9	399995	5	NULL	NULL	0	NULL	strong clinical consideration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the need to address common mental health issues such as depression , given that sleep problems are modifiable and potentially less stigmatizing than mental health problems , assessing and addressing insomnia and nightmares in survivors of interpersonal violence warrants strong clinical consideration and further investigation .
	manualset3
93938	10	399995	5	NULL	NULL	0	NULL	investigation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the need to address common mental health issues such as depression , given that sleep problems are modifiable and potentially less stigmatizing than mental health problems , assessing and addressing insomnia and nightmares in survivors of interpersonal violence warrants strong clinical consideration and further investigation .
	manualset3
93939	1	399996	5	NULL	NULL	0	NULL	precise morphological assessment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the precise morphological assessment of this area of cartilage repair , the cartilage 's biochemical constitution can be determined using biochemical MRI techniques .
	manualset3
93940	2	399996	5	NULL	NULL	0	NULL	area of cartilage repair	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the precise morphological assessment of this area of cartilage repair , the cartilage 's biochemical constitution can be determined using biochemical MRI techniques .
	manualset3
93941	3	399996	5	NULL	NULL	0	NULL	cartilage 's biochemical constitution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the precise morphological assessment of this area of cartilage repair , the cartilage 's biochemical constitution can be determined using biochemical MRI techniques .
	manualset3
93942	4	399996	5	NULL	NULL	0	NULL	biochemical MRI techniques	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the precise morphological assessment of this area of cartilage repair , the cartilage 's biochemical constitution can be determined using biochemical MRI techniques .
	manualset3
93943	1	399997	5	NULL	NULL	0	NULL	adult Fanconi mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In adult Fanconi mice , we showed a reduced proliferation of neural progenitor cells related to apoptosis and accentuated neural stem cells exhaustion with ageing .
	manualset3
93944	2	399997	5	NULL	NULL	0	NULL	proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In adult Fanconi mice , we showed a reduced proliferation of neural progenitor cells related to apoptosis and accentuated neural stem cells exhaustion with ageing .
	manualset3
93945	3	399997	5	NULL	NULL	0	NULL	neural progenitor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In adult Fanconi mice , we showed a reduced proliferation of neural progenitor cells related to apoptosis and accentuated neural stem cells exhaustion with ageing .
	manualset3
93946	4	399997	5	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In adult Fanconi mice , we showed a reduced proliferation of neural progenitor cells related to apoptosis and accentuated neural stem cells exhaustion with ageing .
	manualset3
93947	5	399997	5	NULL	NULL	0	NULL	accentuated neural stem cells exhaustion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In adult Fanconi mice , we showed a reduced proliferation of neural progenitor cells related to apoptosis and accentuated neural stem cells exhaustion with ageing .
	manualset3
98567	6	399997	5	NULL	NULL	0	NULL	ageing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In adult Fanconi mice , we showed a reduced proliferation of neural progenitor cells related to apoptosis and accentuated neural stem cells exhaustion with ageing .
	manualset3
93948	1	399998	5	NULL	NULL	0	NULL	adult mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In adult mice , post-synaptic GFR1 expression did not affect neuron survival following neurotoxic lesion , but it did increase the preservation of striatal dopaminergic innervation .
	manualset3
93949	2	399998	5	NULL	NULL	0	NULL	post-synaptic GFR1 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In adult mice , post-synaptic GFR1 expression did not affect neuron survival following neurotoxic lesion , but it did increase the preservation of striatal dopaminergic innervation .
	manualset3
93950	3	399998	5	NULL	NULL	0	NULL	neuron survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In adult mice , post-synaptic GFR1 expression did not affect neuron survival following neurotoxic lesion , but it did increase the preservation of striatal dopaminergic innervation .
	manualset3
93951	4	399998	5	NULL	NULL	0	NULL	neurotoxic lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In adult mice , post-synaptic GFR1 expression did not affect neuron survival following neurotoxic lesion , but it did increase the preservation of striatal dopaminergic innervation .
	manualset3
93952	5	399998	5	NULL	NULL	0	NULL	preservation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In adult mice , post-synaptic GFR1 expression did not affect neuron survival following neurotoxic lesion , but it did increase the preservation of striatal dopaminergic innervation .
	manualset3
93953	6	399998	5	NULL	NULL	0	NULL	striatal dopaminergic innervation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In adult mice , post-synaptic GFR1 expression did not affect neuron survival following neurotoxic lesion , but it did increase the preservation of striatal dopaminergic innervation .
	manualset3
93954	1	399999	5	NULL	NULL	0	NULL	adult testes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In adult testes , CK2alpha ' and CK2beta subunits are present in spermatocytes .
	manualset3
93955	2	399999	5	NULL	NULL	0	NULL	CK2alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In adult testes , CK2alpha ' and CK2beta subunits are present in spermatocytes .
	manualset3
93956	3	399999	5	NULL	NULL	0	NULL	CK2beta subunits	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In adult testes , CK2alpha ' and CK2beta subunits are present in spermatocytes .
	manualset3
93957	4	399999	5	NULL	NULL	0	NULL	spermatocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In adult testes , CK2alpha ' and CK2beta subunits are present in spermatocytes .
	manualset3
93958	1	400000	5	NULL	NULL	0	NULL	aged human skin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In aged human skin , wound healing rates decrease and cellular damage by reactive oxygen species ( ROS ) accumulates .
	manualset3
93959	2	400000	5	NULL	NULL	0	NULL	wound healing rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In aged human skin , wound healing rates decrease and cellular damage by reactive oxygen species ( ROS ) accumulates .
	manualset3
93961	3	400000	5	NULL	NULL	0	NULL	cellular damage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In aged human skin , wound healing rates decrease and cellular damage by reactive oxygen species ( ROS ) accumulates .
	manualset3
93962	4	400000	5	NULL	NULL	0	NULL	 reactive oxygen species ( ROS )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In aged human skin , wound healing rates decrease and cellular damage by reactive oxygen species ( ROS ) accumulates .
	manualset3
93963	1	400001	5	NULL	NULL	0	NULL	Variations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Variations of oxygen concentration inside incubators ) .
	manualset3
93964	2	400001	5	NULL	NULL	0	NULL	oxygen concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Variations of oxygen concentration inside incubators ) .
	manualset3
93965	3	400001	5	NULL	NULL	0	NULL	incubators	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( Variations of oxygen concentration inside incubators ) .
	manualset3
93966	1	400002	5	NULL	NULL	0	NULL	experimental data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In agreement with experimental data on CEA synthesis in fetal bronchial cell lines , these findings indicate that interstitial lung disorders may induce abnormal CEA-like substance expression .
	manualset3
93967	2	400002	5	NULL	NULL	0	NULL	CEA synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In agreement with experimental data on CEA synthesis in fetal bronchial cell lines , these findings indicate that interstitial lung disorders may induce abnormal CEA-like substance expression .
	manualset3
93968	3	400002	5	NULL	NULL	0	NULL	fetal bronchial cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In agreement with experimental data on CEA synthesis in fetal bronchial cell lines , these findings indicate that interstitial lung disorders may induce abnormal CEA-like substance expression .
	manualset3
93969	4	400002	5	NULL	NULL	0	NULL	interstitial lung disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In agreement with experimental data on CEA synthesis in fetal bronchial cell lines , these findings indicate that interstitial lung disorders may induce abnormal CEA-like substance expression .
	manualset3
93970	5	400002	5	NULL	NULL	0	NULL	abnormal CEA-like substance expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In agreement with experimental data on CEA synthesis in fetal bronchial cell lines , these findings indicate that interstitial lung disorders may induce abnormal CEA-like substance expression .
	manualset3
93971	1	400003	5	NULL	NULL	0	NULL	previous reports	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In agreement with previous reports , indicating that Sec61p displays the majority of the ER ribosome binding activity , we observed that Sec61p is shielded from proteolytic digestion by native , bound ribosomes .
	manualset3
93972	2	400003	5	NULL	NULL	0	NULL	Sec61p	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In agreement with previous reports , indicating that Sec61p displays the majority of the ER ribosome binding activity , we observed that Sec61p is shielded from proteolytic digestion by native , bound ribosomes .
	manualset3
93973	3	400003	5	NULL	NULL	0	NULL	ER ribosome binding activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In agreement with previous reports , indicating that Sec61p displays the majority of the ER ribosome binding activity , we observed that Sec61p is shielded from proteolytic digestion by native , bound ribosomes .
	manualset3
93974	4	400003	5	NULL	NULL	0	NULL	Sec61p	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In agreement with previous reports , indicating that Sec61p displays the majority of the ER ribosome binding activity , we observed that Sec61p is shielded from proteolytic digestion by native , bound ribosomes .
	manualset3
93975	5	400003	5	NULL	NULL	0	NULL	proteolytic digestion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In agreement with previous reports , indicating that Sec61p displays the majority of the ER ribosome binding activity , we observed that Sec61p is shielded from proteolytic digestion by native , bound ribosomes .
	manualset3
93976	6	400003	5	NULL	NULL	0	NULL	native , bound ribosomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In agreement with previous reports , indicating that Sec61p displays the majority of the ER ribosome binding activity , we observed that Sec61p is shielded from proteolytic digestion by native , bound ribosomes .
	manualset3
93977	1	400004	5	NULL	NULL	0	NULL	interpretation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In agreement with this interpretation , an oligosaccharide analysis indicated that 6-sulfo sialyl Lewis X , a major L-selectin ligand sulfated glycan , is almost completely abrogated in the double-deficient mice .
	manualset3
93978	2	400004	5	NULL	NULL	0	NULL	oligosaccharide analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In agreement with this interpretation , an oligosaccharide analysis indicated that 6-sulfo sialyl Lewis X , a major L-selectin ligand sulfated glycan , is almost completely abrogated in the double-deficient mice .
	manualset3
93979	3	400004	5	NULL	NULL	0	NULL	6-sulfo sialyl Lewis X , a major L-selectin ligand sulfated glycan	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In agreement with this interpretation , an oligosaccharide analysis indicated that 6-sulfo sialyl Lewis X , a major L-selectin ligand sulfated glycan , is almost completely abrogated in the double-deficient mice .
	manualset3
93980	4	400004	5	NULL	NULL	0	NULL	double-deficient mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In agreement with this interpretation , an oligosaccharide analysis indicated that 6-sulfo sialyl Lewis X , a major L-selectin ligand sulfated glycan , is almost completely abrogated in the double-deficient mice .
	manualset3
93981	1	400005	5	NULL	NULL	0	NULL	alcoholic women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In alcoholic women the HDL2 mass was increased by 63 % ( P & lt ; 0.01 ) on admission and normalized ( P & lt ; 0.01 ) during abstention .
	manualset3
93982	2	400005	5	NULL	NULL	NULL	NULL	HDL2 mass	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In alcoholic women the HDL2 mass was increased by 63 % ( P & lt ; 0.01 ) on admission and normalized ( P & lt ; 0.01 ) during abstention .
	manualset3
93983	3	400005	5	NULL	NULL	0	NULL	63 % ( P & lt ; 0.01 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In alcoholic women the HDL2 mass was increased by 63 % ( P & lt ; 0.01 ) on admission and normalized ( P & lt ; 0.01 ) during abstention .
	manualset3
93984	4	400005	5	NULL	NULL	0	NULL	admission	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In alcoholic women the HDL2 mass was increased by 63 % ( P & lt ; 0.01 ) on admission and normalized ( P & lt ; 0.01 ) during abstention .
	manualset3
93985	5	400005	5	NULL	NULL	0	NULL	( P & lt ; 0.01 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In alcoholic women the HDL2 mass was increased by 63 % ( P & lt ; 0.01 ) on admission and normalized ( P & lt ; 0.01 ) during abstention .
	manualset3
93986	6	400005	5	NULL	NULL	0	NULL	abstention	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In alcoholic women the HDL2 mass was increased by 63 % ( P & lt ; 0.01 ) on admission and normalized ( P & lt ; 0.01 ) during abstention .
	manualset3
93987	1	400006	5	NULL	NULL	0	NULL	1-5-year-old children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In all , 1-5-year-old children from the Growth , Exercise and Nutrition Epidemiological Study in preSchoolers ( GENESIS ) study ( N = 1980 ) and 11-18-year-old Greek adolescents ( N = 949 ) were measured for adiposity-related phenotypes and genotyped at the FTO single-nucleotide polymorphism ( SNP ) marker , rs17817449 .
	manualset3
93988	2	400006	5	NULL	NULL	NULL	NULL	Growth , Exercise and Nutrition Epidemiological Study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In all , 1-5-year-old children from the Growth , Exercise and Nutrition Epidemiological Study in preSchoolers ( GENESIS ) study ( N = 1980 ) and 11-18-year-old Greek adolescents ( N = 949 ) were measured for adiposity-related phenotypes and genotyped at the FTO single-nucleotide polymorphism ( SNP ) marker , rs17817449 .
	manualset3
93991	3	400006	5	NULL	NULL	NULL	NULL	preSchoolers	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In all , 1-5-year-old children from the Growth , Exercise and Nutrition Epidemiological Study in preSchoolers ( GENESIS ) study ( N = 1980 ) and 11-18-year-old Greek adolescents ( N = 949 ) were measured for adiposity-related phenotypes and genotyped at the FTO single-nucleotide polymorphism ( SNP ) marker , rs17817449 .
	manualset3
93992	4	400006	5	NULL	NULL	0	NULL	( GENESIS ) study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In all , 1-5-year-old children from the Growth , Exercise and Nutrition Epidemiological Study in preSchoolers ( GENESIS ) study ( N = 1980 ) and 11-18-year-old Greek adolescents ( N = 949 ) were measured for adiposity-related phenotypes and genotyped at the FTO single-nucleotide polymorphism ( SNP ) marker , rs17817449 .
	manualset3
93993	5	400006	5	NULL	NULL	0	NULL	N = 1980	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In all , 1-5-year-old children from the Growth , Exercise and Nutrition Epidemiological Study in preSchoolers ( GENESIS ) study ( N = 1980 ) and 11-18-year-old Greek adolescents ( N = 949 ) were measured for adiposity-related phenotypes and genotyped at the FTO single-nucleotide polymorphism ( SNP ) marker , rs17817449 .
	manualset3
93994	6	400006	5	NULL	NULL	0	NULL	11-18-year-old Greek adolescents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In all , 1-5-year-old children from the Growth , Exercise and Nutrition Epidemiological Study in preSchoolers ( GENESIS ) study ( N = 1980 ) and 11-18-year-old Greek adolescents ( N = 949 ) were measured for adiposity-related phenotypes and genotyped at the FTO single-nucleotide polymorphism ( SNP ) marker , rs17817449 .
	manualset3
93995	7	400006	5	NULL	NULL	0	NULL	N = 949	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In all , 1-5-year-old children from the Growth , Exercise and Nutrition Epidemiological Study in preSchoolers ( GENESIS ) study ( N = 1980 ) and 11-18-year-old Greek adolescents ( N = 949 ) were measured for adiposity-related phenotypes and genotyped at the FTO single-nucleotide polymorphism ( SNP ) marker , rs17817449 .
	manualset3
93996	8	400006	5	NULL	NULL	NULL	NULL	adiposity-related phenotypes	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In all , 1-5-year-old children from the Growth , Exercise and Nutrition Epidemiological Study in preSchoolers ( GENESIS ) study ( N = 1980 ) and 11-18-year-old Greek adolescents ( N = 949 ) were measured for adiposity-related phenotypes and genotyped at the FTO single-nucleotide polymorphism ( SNP ) marker , rs17817449 .
	manualset3
93997	9	400006	5	NULL	NULL	0	NULL	FTO single-nucleotide polymorphism ( SNP ) marker , rs17817449	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In all , 1-5-year-old children from the Growth , Exercise and Nutrition Epidemiological Study in preSchoolers ( GENESIS ) study ( N = 1980 ) and 11-18-year-old Greek adolescents ( N = 949 ) were measured for adiposity-related phenotypes and genotyped at the FTO single-nucleotide polymorphism ( SNP ) marker , rs17817449 .
	manualset3
93999	1	400007	5	NULL	NULL	0	NULL	152 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In all , 152 patients with a NRS3 and undergoing elective major GI surgery were randomized between IN or isocaloric-isonitrogenous nutrition ( ICN ) given for 5 days preoperatively .
	manualset3
94000	2	400007	5	NULL	NULL	0	NULL	NRS3	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In all , 152 patients with a NRS3 and undergoing elective major GI surgery were randomized between IN or isocaloric-isonitrogenous nutrition ( ICN ) given for 5 days preoperatively .
	manualset3
94001	3	400007	5	NULL	NULL	0	NULL	elective major GI surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In all , 152 patients with a NRS3 and undergoing elective major GI surgery were randomized between IN or isocaloric-isonitrogenous nutrition ( ICN ) given for 5 days preoperatively .
	manualset3
94002	4	400007	5	NULL	NULL	0	NULL	IN	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	In all , 152 patients with a NRS3 and undergoing elective major GI surgery were randomized between IN or isocaloric-isonitrogenous nutrition ( ICN ) given for 5 days preoperatively .
	manualset3
94003	5	400007	5	NULL	NULL	0	NULL	isocaloric-isonitrogenous nutrition ( ICN )	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	In all , 152 patients with a NRS3 and undergoing elective major GI surgery were randomized between IN or isocaloric-isonitrogenous nutrition ( ICN ) given for 5 days preoperatively .
	manualset3
94004	6	400007	5	NULL	NULL	0	NULL	5 days	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In all , 152 patients with a NRS3 and undergoing elective major GI surgery were randomized between IN or isocaloric-isonitrogenous nutrition ( ICN ) given for 5 days preoperatively .
	manualset3
94005	1	400008	5	NULL	NULL	0	NULL	16 of the 18 tumor samples	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In all , 16 of the 18 tumor samples expressed increased levels of nm23 H1/NDPKA mRNA as compared with those measured in normal tissue .
	manualset3
94006	2	400008	5	NULL	NULL	0	NULL	increased levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In all , 16 of the 18 tumor samples expressed increased levels of nm23 H1/NDPKA mRNA as compared with those measured in normal tissue .
	manualset3
94007	3	400008	5	NULL	NULL	0	NULL	nm23 H1/NDPKA mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In all , 16 of the 18 tumor samples expressed increased levels of nm23 H1/NDPKA mRNA as compared with those measured in normal tissue .
	manualset3
94008	4	400008	5	NULL	NULL	0	NULL	normal tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In all , 16 of the 18 tumor samples expressed increased levels of nm23 H1/NDPKA mRNA as compared with those measured in normal tissue .
	manualset3
94009	1	400009	5	NULL	NULL	NULL	NULL	cases	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In all cases , including 1 in which the newborn was D negative , a sharp increment in the anti-D titer was observed after delivery .
	manualset3
94010	2	400009	5	NULL	NULL	0	NULL	1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In all cases , including 1 in which the newborn was D negative , a sharp increment in the anti-D titer was observed after delivery .
	manualset3
94011	3	400009	5	NULL	NULL	0	NULL	newborn	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In all cases , including 1 in which the newborn was D negative , a sharp increment in the anti-D titer was observed after delivery .
	manualset3
94012	4	400009	5	NULL	NULL	0	NULL	D negative	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In all cases , including 1 in which the newborn was D negative , a sharp increment in the anti-D titer was observed after delivery .
	manualset3
94013	5	400009	5	NULL	NULL	0	NULL	anti-D titer	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In all cases , including 1 in which the newborn was D negative , a sharp increment in the anti-D titer was observed after delivery .
	manualset3
94014	6	400009	5	NULL	NULL	0	NULL	delivery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In all cases , including 1 in which the newborn was D negative , a sharp increment in the anti-D titer was observed after delivery .
	manualset3
94015	1	400010	5	NULL	NULL	0	NULL	cases	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In all cases , the conjugate stability was shear dependent over a 100-fold range ( 0.04 to 4.0 dynes/cm2 ) .
	manualset3
94016	2	400010	5	NULL	NULL	0	NULL	conjugate stability	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In all cases , the conjugate stability was shear dependent over a 100-fold range ( 0.04 to 4.0 dynes/cm2 ) .
	manualset3
94017	3	400010	5	NULL	NULL	0	NULL	100-fold range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In all cases , the conjugate stability was shear dependent over a 100-fold range ( 0.04 to 4.0 dynes/cm2 ) .
	manualset3
94018	4	400010	5	NULL	NULL	0	NULL	( 0.04 to 4.0 dynes/cm2 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In all cases , the conjugate stability was shear dependent over a 100-fold range ( 0.04 to 4.0 dynes/cm2 ) .
	manualset3
94019	1	400011	5	NULL	NULL	0	NULL	gingival specimens	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In all gingival specimens examined , cathepsin G and medullasin were found mainly in neutrophil-like cells and partly in macrophage-like cells .
	manualset3
94020	2	400011	5	NULL	NULL	0	NULL	cathepsin G	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In all gingival specimens examined , cathepsin G and medullasin were found mainly in neutrophil-like cells and partly in macrophage-like cells .
	manualset3
94021	3	400011	5	NULL	NULL	0	NULL	medullasin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In all gingival specimens examined , cathepsin G and medullasin were found mainly in neutrophil-like cells and partly in macrophage-like cells .
	manualset3
94022	4	400011	5	NULL	NULL	0	NULL	neutrophil-like cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In all gingival specimens examined , cathepsin G and medullasin were found mainly in neutrophil-like cells and partly in macrophage-like cells .
	manualset3
94023	5	400011	5	NULL	NULL	0	NULL	macrophage-like cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In all gingival specimens examined , cathepsin G and medullasin were found mainly in neutrophil-like cells and partly in macrophage-like cells .
	manualset3
94024	1	400012	5	NULL	NULL	0	NULL	lymphoid tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In all lymphoid tissues , Gl-1 strongly stained certain distinct regions that are occupied by dendritic cells and by macrophages .
	manualset3
94025	2	400012	5	NULL	NULL	0	NULL	Gl-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In all lymphoid tissues , Gl-1 strongly stained certain distinct regions that are occupied by dendritic cells and by macrophages .
	manualset3
94026	3	400012	5	NULL	NULL	0	NULL	distinct regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In all lymphoid tissues , Gl-1 strongly stained certain distinct regions that are occupied by dendritic cells and by macrophages .
	manualset3
94027	4	400012	5	NULL	NULL	0	NULL	dendritic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In all lymphoid tissues , Gl-1 strongly stained certain distinct regions that are occupied by dendritic cells and by macrophages .
	manualset3
94028	5	400012	5	NULL	NULL	0	NULL	macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In all lymphoid tissues , Gl-1 strongly stained certain distinct regions that are occupied by dendritic cells and by macrophages .
	manualset3
94029	1	400013	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In all patients , the repeat 67Ga lung scans remained normal or showed no change after bronchoscopy and BAL .
	manualset3
94030	2	400013	5	NULL	NULL	0	NULL	repeat 67Ga lung scans	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In all patients , the repeat 67Ga lung scans remained normal or showed no change after bronchoscopy and BAL .
	manualset3
94031	3	400013	5	NULL	NULL	0	NULL	bronchoscopy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In all patients , the repeat 67Ga lung scans remained normal or showed no change after bronchoscopy and BAL .
	manualset3
94032	4	400013	5	NULL	NULL	0	NULL	BAL	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In all patients , the repeat 67Ga lung scans remained normal or showed no change after bronchoscopy and BAL .
	manualset3
94033	1	400014	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In all patients the range of motion of the elbow improved significantly .
	manualset3
94034	2	400014	5	NULL	NULL	0	NULL	range of motion	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In all patients the range of motion of the elbow improved significantly .
	manualset3
94036	3	400014	5	NULL	NULL	0	NULL	elbow	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In all patients the range of motion of the elbow improved significantly .
	manualset3
94038	1	400015	5	NULL	NULL	0	NULL	treatment groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In all treatment groups , reduced weights of seminal vesicle , prostate and epididymis , and degeneration/necrosis of the pachytene spermatocytes in stages VII or VIII seminiferous tubules , were dose-relatedly observed .
	manualset3
94040	2	400015	5	NULL	NULL	0	NULL	reduced weights	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In all treatment groups , reduced weights of seminal vesicle , prostate and epididymis , and degeneration/necrosis of the pachytene spermatocytes in stages VII or VIII seminiferous tubules , were dose-relatedly observed .
	manualset3
94042	3	400015	5	NULL	NULL	0	NULL	seminal vesicle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In all treatment groups , reduced weights of seminal vesicle , prostate and epididymis , and degeneration/necrosis of the pachytene spermatocytes in stages VII or VIII seminiferous tubules , were dose-relatedly observed .
	manualset3
94043	4	400015	5	NULL	NULL	0	NULL	prostate	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In all treatment groups , reduced weights of seminal vesicle , prostate and epididymis , and degeneration/necrosis of the pachytene spermatocytes in stages VII or VIII seminiferous tubules , were dose-relatedly observed .
	manualset3
94044	5	400015	5	NULL	NULL	0	NULL	epididymis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In all treatment groups , reduced weights of seminal vesicle , prostate and epididymis , and degeneration/necrosis of the pachytene spermatocytes in stages VII or VIII seminiferous tubules , were dose-relatedly observed .
	manualset3
94045	6	400015	5	NULL	NULL	0	NULL	degeneration/necrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In all treatment groups , reduced weights of seminal vesicle , prostate and epididymis , and degeneration/necrosis of the pachytene spermatocytes in stages VII or VIII seminiferous tubules , were dose-relatedly observed .
	manualset3
94046	7	400015	5	NULL	NULL	0	NULL	pachytene spermatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In all treatment groups , reduced weights of seminal vesicle , prostate and epididymis , and degeneration/necrosis of the pachytene spermatocytes in stages VII or VIII seminiferous tubules , were dose-relatedly observed .
	manualset3
94047	8	400015	5	NULL	NULL	0	NULL	stages VII or VIII seminiferous tubules	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In all treatment groups , reduced weights of seminal vesicle , prostate and epididymis , and degeneration/necrosis of the pachytene spermatocytes in stages VII or VIII seminiferous tubules , were dose-relatedly observed .
	manualset3
94048	1	400016	5	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In all the cases , although the inhibitory effect of PSC was evident at both doses , only PSC30 exhibited statistical significance .
	manualset3
94049	2	400016	5	NULL	NULL	0	NULL	inhibitory effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In all the cases , although the inhibitory effect of PSC was evident at both doses , only PSC30 exhibited statistical significance .
	manualset3
94050	3	400016	5	NULL	NULL	0	NULL	PSC 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In all the cases , although the inhibitory effect of PSC was evident at both doses , only PSC30 exhibited statistical significance .
	manualset3
94051	4	400016	5	NULL	NULL	0	NULL	doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In all the cases , although the inhibitory effect of PSC was evident at both doses , only PSC30 exhibited statistical significance .
	manualset3
94052	5	400016	5	NULL	NULL	0	NULL	PSC30 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In all the cases , although the inhibitory effect of PSC was evident at both doses , only PSC30 exhibited statistical significance .
	manualset3
94053	6	400016	5	NULL	NULL	0	NULL	statistical significance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In all the cases , although the inhibitory effect of PSC was evident at both doses , only PSC30 exhibited statistical significance .
	manualset3
94054	1	400017	5	NULL	NULL	0	NULL	cases	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In all the other cases detachment of the germinal membrane and subsequent reduction in size was observed , with a more or less complete solidification of the cyst and reduction of serology titers .
	manualset3
94055	2	400017	5	NULL	NULL	0	NULL	detachment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In all the other cases detachment of the germinal membrane and subsequent reduction in size was observed , with a more or less complete solidification of the cyst and reduction of serology titers .
	manualset3
94056	3	400017	5	NULL	NULL	0	NULL	germinal membrane	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In all the other cases detachment of the germinal membrane and subsequent reduction in size was observed , with a more or less complete solidification of the cyst and reduction of serology titers .
	manualset3
94057	4	400017	5	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In all the other cases detachment of the germinal membrane and subsequent reduction in size was observed , with a more or less complete solidification of the cyst and reduction of serology titers .
	manualset3
94058	5	400017	5	NULL	NULL	0	NULL	size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In all the other cases detachment of the germinal membrane and subsequent reduction in size was observed , with a more or less complete solidification of the cyst and reduction of serology titers .
	manualset3
94059	6	400017	5	NULL	NULL	0	NULL	more or less complete solidification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In all the other cases detachment of the germinal membrane and subsequent reduction in size was observed , with a more or less complete solidification of the cyst and reduction of serology titers .
	manualset3
94060	7	400017	5	NULL	NULL	0	NULL	cyst 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In all the other cases detachment of the germinal membrane and subsequent reduction in size was observed , with a more or less complete solidification of the cyst and reduction of serology titers .
	manualset3
94061	8	400017	5	NULL	NULL	0	NULL	reduction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In all the other cases detachment of the germinal membrane and subsequent reduction in size was observed , with a more or less complete solidification of the cyst and reduction of serology titers .
	manualset3
94062	9	400017	5	NULL	NULL	0	NULL	serology titers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In all the other cases detachment of the germinal membrane and subsequent reduction in size was observed , with a more or less complete solidification of the cyst and reduction of serology titers .
	manualset3
94063	1	400018	5	NULL	NULL	0	NULL	cases	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In almost all cases , the MeMAD is well separated from the randomized outcome .
	manualset3
94064	2	400018	5	NULL	NULL	0	NULL	MeMAD	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In almost all cases , the MeMAD is well separated from the randomized outcome .
	manualset3
94065	3	400018	5	NULL	NULL	0	NULL	randomized outcome	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In almost all cases , the MeMAD is well separated from the randomized outcome .
	manualset3
94066	1	400019	5	NULL	NULL	0	NULL	amphibian tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In amphibian and avian tissues multiple forms of the enzyme seem to be present which differ for the substrate concentration at half-maximal velocity ( S0 .5 ) ; the concentration of nucleotide effector which affords half-maximal protection at 37 degrees C ( P0 .5 ) ; and the Hill coefficient for monophosphate donor .
	manualset3
94067	2	400019	5	NULL	NULL	0	NULL	avian tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In amphibian and avian tissues multiple forms of the enzyme seem to be present which differ for the substrate concentration at half-maximal velocity ( S0 .5 ) ; the concentration of nucleotide effector which affords half-maximal protection at 37 degrees C ( P0 .5 ) ; and the Hill coefficient for monophosphate donor .
	manualset3
94068	3	400019	5	NULL	NULL	0	NULL	multiple forms of the enzyme	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In amphibian and avian tissues multiple forms of the enzyme seem to be present which differ for the substrate concentration at half-maximal velocity ( S0 .5 ) ; the concentration of nucleotide effector which affords half-maximal protection at 37 degrees C ( P0 .5 ) ; and the Hill coefficient for monophosphate donor .
	manualset3
94069	4	400019	5	NULL	NULL	0	NULL	substrate concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In amphibian and avian tissues multiple forms of the enzyme seem to be present which differ for the substrate concentration at half-maximal velocity ( S0 .5 ) ; the concentration of nucleotide effector which affords half-maximal protection at 37 degrees C ( P0 .5 ) ; and the Hill coefficient for monophosphate donor .
	manualset3
94070	5	400019	5	NULL	NULL	0	NULL	half-maximal velocity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In amphibian and avian tissues multiple forms of the enzyme seem to be present which differ for the substrate concentration at half-maximal velocity ( S0 .5 ) ; the concentration of nucleotide effector which affords half-maximal protection at 37 degrees C ( P0 .5 ) ; and the Hill coefficient for monophosphate donor .
	manualset3
94071	6	400019	5	NULL	NULL	0	NULL	S0 .5	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In amphibian and avian tissues multiple forms of the enzyme seem to be present which differ for the substrate concentration at half-maximal velocity ( S0 .5 ) ; the concentration of nucleotide effector which affords half-maximal protection at 37 degrees C ( P0 .5 ) ; and the Hill coefficient for monophosphate donor .
	manualset3
94072	7	400019	5	NULL	NULL	0	NULL	concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In amphibian and avian tissues multiple forms of the enzyme seem to be present which differ for the substrate concentration at half-maximal velocity ( S0 .5 ) ; the concentration of nucleotide effector which affords half-maximal protection at 37 degrees C ( P0 .5 ) ; and the Hill coefficient for monophosphate donor .
	manualset3
94073	8	400019	5	NULL	NULL	0	NULL	nucleotide effector	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In amphibian and avian tissues multiple forms of the enzyme seem to be present which differ for the substrate concentration at half-maximal velocity ( S0 .5 ) ; the concentration of nucleotide effector which affords half-maximal protection at 37 degrees C ( P0 .5 ) ; and the Hill coefficient for monophosphate donor .
	manualset3
94074	9	400019	5	NULL	NULL	0	NULL	half-maximal protection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In amphibian and avian tissues multiple forms of the enzyme seem to be present which differ for the substrate concentration at half-maximal velocity ( S0 .5 ) ; the concentration of nucleotide effector which affords half-maximal protection at 37 degrees C ( P0 .5 ) ; and the Hill coefficient for monophosphate donor .
	manualset3
94075	10	400019	5	NULL	NULL	0	NULL	37 degrees C	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In amphibian and avian tissues multiple forms of the enzyme seem to be present which differ for the substrate concentration at half-maximal velocity ( S0 .5 ) ; the concentration of nucleotide effector which affords half-maximal protection at 37 degrees C ( P0 .5 ) ; and the Hill coefficient for monophosphate donor .
	manualset3
94076	11	400019	5	NULL	NULL	0	NULL	P0 .5 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In amphibian and avian tissues multiple forms of the enzyme seem to be present which differ for the substrate concentration at half-maximal velocity ( S0 .5 ) ; the concentration of nucleotide effector which affords half-maximal protection at 37 degrees C ( P0 .5 ) ; and the Hill coefficient for monophosphate donor .
	manualset3
94077	12	400019	5	NULL	NULL	0	NULL	Hill coefficient	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In amphibian and avian tissues multiple forms of the enzyme seem to be present which differ for the substrate concentration at half-maximal velocity ( S0 .5 ) ; the concentration of nucleotide effector which affords half-maximal protection at 37 degrees C ( P0 .5 ) ; and the Hill coefficient for monophosphate donor .
	manualset3
94078	13	400019	5	NULL	NULL	0	NULL	monophosphate donor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In amphibian and avian tissues multiple forms of the enzyme seem to be present which differ for the substrate concentration at half-maximal velocity ( S0 .5 ) ; the concentration of nucleotide effector which affords half-maximal protection at 37 degrees C ( P0 .5 ) ; and the Hill coefficient for monophosphate donor .
	manualset3
94079	1	400020	5	NULL	NULL	0	NULL	acute toxicity study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In an acute toxicity study using Sprague-Dawley rats , the median lethal dose ( LD50 ) of Yumijangquebo was greater than 2000 mg/kg , and we found no pathological changes in macroscopic examination by necropsy of rats treated with Yumijangquebo .
	manualset3
94080	2	400020	5	NULL	NULL	0	NULL	Sprague-Dawley rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In an acute toxicity study using Sprague-Dawley rats , the median lethal dose ( LD50 ) of Yumijangquebo was greater than 2000 mg/kg , and we found no pathological changes in macroscopic examination by necropsy of rats treated with Yumijangquebo .
	manualset3
94081	3	400020	5	NULL	NULL	0	NULL	median lethal dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In an acute toxicity study using Sprague-Dawley rats , the median lethal dose ( LD50 ) of Yumijangquebo was greater than 2000 mg/kg , and we found no pathological changes in macroscopic examination by necropsy of rats treated with Yumijangquebo .
	manualset3
94082	4	400020	5	NULL	NULL	0	NULL	( LD50 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In an acute toxicity study using Sprague-Dawley rats , the median lethal dose ( LD50 ) of Yumijangquebo was greater than 2000 mg/kg , and we found no pathological changes in macroscopic examination by necropsy of rats treated with Yumijangquebo .
	manualset3
94083	5	400020	5	NULL	NULL	NULL	NULL	Yumijangquebo	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In an acute toxicity study using Sprague-Dawley rats , the median lethal dose ( LD50 ) of Yumijangquebo was greater than 2000 mg/kg , and we found no pathological changes in macroscopic examination by necropsy of rats treated with Yumijangquebo .
	manualset3
94084	6	400020	5	NULL	NULL	0	NULL	2000 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In an acute toxicity study using Sprague-Dawley rats , the median lethal dose ( LD50 ) of Yumijangquebo was greater than 2000 mg/kg , and we found no pathological changes in macroscopic examination by necropsy of rats treated with Yumijangquebo .
	manualset3
94085	7	400020	5	NULL	NULL	0	NULL	pathological changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In an acute toxicity study using Sprague-Dawley rats , the median lethal dose ( LD50 ) of Yumijangquebo was greater than 2000 mg/kg , and we found no pathological changes in macroscopic examination by necropsy of rats treated with Yumijangquebo .
	manualset3
94086	8	400020	5	NULL	NULL	0	NULL	macroscopic examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In an acute toxicity study using Sprague-Dawley rats , the median lethal dose ( LD50 ) of Yumijangquebo was greater than 2000 mg/kg , and we found no pathological changes in macroscopic examination by necropsy of rats treated with Yumijangquebo .
	manualset3
94087	9	400020	5	NULL	NULL	0	NULL	necropsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In an acute toxicity study using Sprague-Dawley rats , the median lethal dose ( LD50 ) of Yumijangquebo was greater than 2000 mg/kg , and we found no pathological changes in macroscopic examination by necropsy of rats treated with Yumijangquebo .
	manualset3
94088	10	400020	5	NULL	NULL	NULL	NULL	rats treated with Yumijangquebo	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In an acute toxicity study using Sprague-Dawley rats , the median lethal dose ( LD50 ) of Yumijangquebo was greater than 2000 mg/kg , and we found no pathological changes in macroscopic examination by necropsy of rats treated with Yumijangquebo .
	manualset3
94089	1	400021	5	NULL	NULL	0	NULL	adult intensive care unit ( ICU ) population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In an adult intensive care unit ( ICU ) population , we identify a specific and important question-can PCT accurately distinguish sepsis in patients with systemic inflammatory response syndrome ( SIRS ) who have a suspected infection ?
	manualset3
94090	2	400021	5	NULL	NULL	0	NULL	specific and important question	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In an adult intensive care unit ( ICU ) population , we identify a specific and important question-can PCT accurately distinguish sepsis in patients with systemic inflammatory response syndrome ( SIRS ) who have a suspected infection ?
	manualset3
94091	3	400021	5	NULL	NULL	0	NULL	PCT	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In an adult intensive care unit ( ICU ) population , we identify a specific and important question-can PCT accurately distinguish sepsis in patients with systemic inflammatory response syndrome ( SIRS ) who have a suspected infection ?
	manualset3
94092	4	400021	5	NULL	NULL	0	NULL	sepsis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In an adult intensive care unit ( ICU ) population , we identify a specific and important question-can PCT accurately distinguish sepsis in patients with systemic inflammatory response syndrome ( SIRS ) who have a suspected infection ?
	manualset3
94093	5	400021	5	NULL	NULL	0	NULL	patients with systemic inflammatory response syndrome ( SIRS )	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In an adult intensive care unit ( ICU ) population , we identify a specific and important question-can PCT accurately distinguish sepsis in patients with systemic inflammatory response syndrome ( SIRS ) who have a suspected infection ?
	manualset3
94094	6	400021	5	NULL	NULL	0	NULL	infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In an adult intensive care unit ( ICU ) population , we identify a specific and important question-can PCT accurately distinguish sepsis in patients with systemic inflammatory response syndrome ( SIRS ) who have a suspected infection ?
	manualset3
94095	1	400022	5	NULL	NULL	0	NULL	discover	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to discover the cause of lysozyme resistance , we identified a gene , oatA , in Staphylococcus aureus .
	manualset3
94096	2	400022	5	NULL	NULL	0	NULL	lysozyme resistance	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to discover the cause of lysozyme resistance , we identified a gene , oatA , in Staphylococcus aureus .
	manualset3
94097	3	400022	5	NULL	NULL	0	NULL	gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to discover the cause of lysozyme resistance , we identified a gene , oatA , in Staphylococcus aureus .
	manualset3
94098	4	400022	5	NULL	NULL	0	NULL	oatA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to discover the cause of lysozyme resistance , we identified a gene , oatA , in Staphylococcus aureus .
	manualset3
94099	5	400022	5	NULL	NULL	0	NULL	Staphylococcus aureus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to discover the cause of lysozyme resistance , we identified a gene , oatA , in Staphylococcus aureus .
	manualset3
94100	1	400023	5	NULL	NULL	0	NULL	significance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to elucidate the significance of ACTH independent mechanisms in the regulation of cortisol secretion in man , the dynamics of plasma ACTH and cortisol levels were studied in response to different stimuli .
	manualset3
94101	2	400023	5	NULL	NULL	0	NULL	ACTH independent mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to elucidate the significance of ACTH independent mechanisms in the regulation of cortisol secretion in man , the dynamics of plasma ACTH and cortisol levels were studied in response to different stimuli .
	manualset3
94102	3	400023	5	NULL	NULL	0	NULL	regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to elucidate the significance of ACTH independent mechanisms in the regulation of cortisol secretion in man , the dynamics of plasma ACTH and cortisol levels were studied in response to different stimuli .
	manualset3
94103	4	400023	5	NULL	NULL	0	NULL	cortisol secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to elucidate the significance of ACTH independent mechanisms in the regulation of cortisol secretion in man , the dynamics of plasma ACTH and cortisol levels were studied in response to different stimuli .
	manualset3
94104	5	400023	5	NULL	NULL	NULL	NULL	man	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In an attempt to elucidate the significance of ACTH independent mechanisms in the regulation of cortisol secretion in man , the dynamics of plasma ACTH and cortisol levels were studied in response to different stimuli .
	manualset3
94105	6	400023	5	NULL	NULL	0	NULL	dynamics	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to elucidate the significance of ACTH independent mechanisms in the regulation of cortisol secretion in man , the dynamics of plasma ACTH and cortisol levels were studied in response to different stimuli .
	manualset3
94106	7	400023	5	NULL	NULL	0	NULL	plasma ACTH 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to elucidate the significance of ACTH independent mechanisms in the regulation of cortisol secretion in man , the dynamics of plasma ACTH and cortisol levels were studied in response to different stimuli .
	manualset3
94107	8	400023	5	NULL	NULL	0	NULL	cortisol levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to elucidate the significance of ACTH independent mechanisms in the regulation of cortisol secretion in man , the dynamics of plasma ACTH and cortisol levels were studied in response to different stimuli .
	manualset3
94108	9	400023	5	NULL	NULL	0	NULL	response to different stimuli	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to elucidate the significance of ACTH independent mechanisms in the regulation of cortisol secretion in man , the dynamics of plasma ACTH and cortisol levels were studied in response to different stimuli .
	manualset3
94109	1	400024	5	NULL	NULL	0	NULL	histological diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Various steps in the histological diagnosis of mediastinobronchopulmonary cancers ) .
	manualset3
94110	2	400024	5	NULL	NULL	0	NULL	 mediastinobronchopulmonary cancers	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Various steps in the histological diagnosis of mediastinobronchopulmonary cancers ) .
	manualset3
94111	1	400025	5	NULL	NULL	0	NULL	utility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to expand the utility of the model Hamiltonian technique developed by Koppel , Domcke , and Cederbaum ( KDC ) ( Adv .
	manualset3
94112	2	400025	5	NULL	NULL	NULL	NULL	model Hamiltonian technique	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In an attempt to expand the utility of the model Hamiltonian technique developed by Koppel , Domcke , and Cederbaum ( KDC ) ( Adv .
	manualset3
94113	3	400025	5	NULL	NULL	NULL	NULL	Koppel , Domcke , and Cederbaum ( KDC )	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In an attempt to expand the utility of the model Hamiltonian technique developed by Koppel , Domcke , and Cederbaum ( KDC ) ( Adv .
	manualset3
94114	1	400026	5	NULL	NULL	NULL	NULL	structural deviation	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In an attempt to find a structural deviation in upper airway anatomy , we performed acoustic echography and cephalometric roentgenograms in 9 male patients with OSA and no clinical evidence of upper airway abnormality .
	manualset3
94115	2	400026	5	NULL	NULL	0	NULL	upper airway anatomy	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to find a structural deviation in upper airway anatomy , we performed acoustic echography and cephalometric roentgenograms in 9 male patients with OSA and no clinical evidence of upper airway abnormality .
	manualset3
94116	3	400026	5	NULL	NULL	NULL	NULL	acoustic echography 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In an attempt to find a structural deviation in upper airway anatomy , we performed acoustic echography and cephalometric roentgenograms in 9 male patients with OSA and no clinical evidence of upper airway abnormality .
	manualset3
94117	4	400026	5	NULL	NULL	0	NULL	cephalometric roentgenograms	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to find a structural deviation in upper airway anatomy , we performed acoustic echography and cephalometric roentgenograms in 9 male patients with OSA and no clinical evidence of upper airway abnormality .
	manualset3
94118	5	400026	5	NULL	NULL	0	NULL	9 male patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to find a structural deviation in upper airway anatomy , we performed acoustic echography and cephalometric roentgenograms in 9 male patients with OSA and no clinical evidence of upper airway abnormality .
	manualset3
94119	6	400026	5	NULL	NULL	0	NULL	OSA	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to find a structural deviation in upper airway anatomy , we performed acoustic echography and cephalometric roentgenograms in 9 male patients with OSA and no clinical evidence of upper airway abnormality .
	manualset3
94120	7	400026	5	NULL	NULL	0	NULL	clinical evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to find a structural deviation in upper airway anatomy , we performed acoustic echography and cephalometric roentgenograms in 9 male patients with OSA and no clinical evidence of upper airway abnormality .
	manualset3
94121	8	400026	5	NULL	NULL	0	NULL	upper airway abnormality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to find a structural deviation in upper airway anatomy , we performed acoustic echography and cephalometric roentgenograms in 9 male patients with OSA and no clinical evidence of upper airway abnormality .
	manualset3
94122	1	400027	5	NULL	NULL	0	NULL	contradictory reports	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to resolve contradictory reports about the effect of right-versus left-hemisphere damage on perception of the Mueller-Lyer illusion , the present study examined judgments of stroke patients using this and several other visual illusions .
	manualset3
94123	2	400027	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to resolve contradictory reports about the effect of right-versus left-hemisphere damage on perception of the Mueller-Lyer illusion , the present study examined judgments of stroke patients using this and several other visual illusions .
	manualset3
94124	3	400027	5	NULL	NULL	0	NULL	right-versus left-hemisphere damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to resolve contradictory reports about the effect of right-versus left-hemisphere damage on perception of the Mueller-Lyer illusion , the present study examined judgments of stroke patients using this and several other visual illusions .
	manualset3
94125	4	400027	5	NULL	NULL	0	NULL	perception 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to resolve contradictory reports about the effect of right-versus left-hemisphere damage on perception of the Mueller-Lyer illusion , the present study examined judgments of stroke patients using this and several other visual illusions .
	manualset3
94126	5	400027	5	NULL	NULL	0	NULL	Mueller-Lyer illusion	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to resolve contradictory reports about the effect of right-versus left-hemisphere damage on perception of the Mueller-Lyer illusion , the present study examined judgments of stroke patients using this and several other visual illusions .
	manualset3
94127	6	400027	5	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to resolve contradictory reports about the effect of right-versus left-hemisphere damage on perception of the Mueller-Lyer illusion , the present study examined judgments of stroke patients using this and several other visual illusions .
	manualset3
94128	7	400027	5	NULL	NULL	0	NULL	judgments 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to resolve contradictory reports about the effect of right-versus left-hemisphere damage on perception of the Mueller-Lyer illusion , the present study examined judgments of stroke patients using this and several other visual illusions .
	manualset3
94129	8	400027	5	NULL	NULL	0	NULL	stroke patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to resolve contradictory reports about the effect of right-versus left-hemisphere damage on perception of the Mueller-Lyer illusion , the present study examined judgments of stroke patients using this and several other visual illusions .
	manualset3
94130	9	400027	5	NULL	NULL	0	NULL	visual illusions	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to resolve contradictory reports about the effect of right-versus left-hemisphere damage on perception of the Mueller-Lyer illusion , the present study examined judgments of stroke patients using this and several other visual illusions .
	manualset3
94131	1	400028	5	NULL	NULL	0	NULL	 early branching metazoan	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In an early branching metazoan , bacterial colonization of the embryo is controlled by maternal antimicrobial peptides .
	manualset3
94132	2	400028	5	NULL	NULL	0	NULL	bacterial colonization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In an early branching metazoan , bacterial colonization of the embryo is controlled by maternal antimicrobial peptides .
	manualset3
94133	3	400028	5	NULL	NULL	0	NULL	embryo	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In an early branching metazoan , bacterial colonization of the embryo is controlled by maternal antimicrobial peptides .
	manualset3
94134	4	400028	5	NULL	NULL	0	NULL	maternal antimicrobial peptides	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In an early branching metazoan , bacterial colonization of the embryo is controlled by maternal antimicrobial peptides .
	manualset3
94135	1	400029	5	NULL	NULL	0	NULL	effort	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In an effort to identify and analyze mutations in the human CBS gene , we have developed a yeast expression system for human CBS .
	manualset3
94136	2	400029	5	NULL	NULL	NULL	NULL	mutations	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In an effort to identify and analyze mutations in the human CBS gene , we have developed a yeast expression system for human CBS .
	manualset3
94137	3	400029	5	NULL	NULL	0	NULL	 human CBS gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In an effort to identify and analyze mutations in the human CBS gene , we have developed a yeast expression system for human CBS .
	manualset3
94138	4	400029	5	NULL	NULL	NULL	NULL	yeast expression system	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In an effort to identify and analyze mutations in the human CBS gene , we have developed a yeast expression system for human CBS .
	manualset3
94139	5	400029	5	NULL	NULL	0	NULL	human CBS	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In an effort to identify and analyze mutations in the human CBS gene , we have developed a yeast expression system for human CBS .
	manualset3
94140	1	400030	5	NULL	NULL	NULL	NULL	functional versatility	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In an effort to judge the functional versatility of RNA and thereby the plausibility that RNA was at one point the basis for life , a statistical chemical approach is adopted .
	manualset3
94141	2	400030	5	NULL	NULL	0	NULL	RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In an effort to judge the functional versatility of RNA and thereby the plausibility that RNA was at one point the basis for life , a statistical chemical approach is adopted .
	manualset3
94142	3	400030	5	NULL	NULL	0	NULL	plausibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In an effort to judge the functional versatility of RNA and thereby the plausibility that RNA was at one point the basis for life , a statistical chemical approach is adopted .
	manualset3
94143	4	400030	5	NULL	NULL	0	NULL	RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In an effort to judge the functional versatility of RNA and thereby the plausibility that RNA was at one point the basis for life , a statistical chemical approach is adopted .
	manualset3
94144	5	400030	5	NULL	NULL	0	NULL	life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In an effort to judge the functional versatility of RNA and thereby the plausibility that RNA was at one point the basis for life , a statistical chemical approach is adopted .
	manualset3
94145	6	400030	5	NULL	NULL	0	NULL	statistical chemical approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In an effort to judge the functional versatility of RNA and thereby the plausibility that RNA was at one point the basis for life , a statistical chemical approach is adopted .
	manualset3
94433	1	400031	5	NULL	NULL	0	NULL	effort	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In an effort to uncover the cathepsin L expression in diverse pathological conditions in human testis , the immunohistochemical localization of cathepsin L was conducted in human testis under diverse male infertility condition including spermatogenic hypoplasia and testis cancer .
	manualset3
94434	2	400031	5	NULL	NULL	0	NULL	cathepsin L expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In an effort to uncover the cathepsin L expression in diverse pathological conditions in human testis , the immunohistochemical localization of cathepsin L was conducted in human testis under diverse male infertility condition including spermatogenic hypoplasia and testis cancer .
	manualset3
94436	3	400031	5	NULL	NULL	0	NULL	diverse pathological conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In an effort to uncover the cathepsin L expression in diverse pathological conditions in human testis , the immunohistochemical localization of cathepsin L was conducted in human testis under diverse male infertility condition including spermatogenic hypoplasia and testis cancer .
	manualset3
94437	4	400031	5	NULL	NULL	0	NULL	human testis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In an effort to uncover the cathepsin L expression in diverse pathological conditions in human testis , the immunohistochemical localization of cathepsin L was conducted in human testis under diverse male infertility condition including spermatogenic hypoplasia and testis cancer .
	manualset3
94439	5	400031	5	NULL	NULL	NULL	NULL	immunohistochemical localization	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In an effort to uncover the cathepsin L expression in diverse pathological conditions in human testis , the immunohistochemical localization of cathepsin L was conducted in human testis under diverse male infertility condition including spermatogenic hypoplasia and testis cancer .
	manualset3
94441	6	400031	5	NULL	NULL	0	NULL	cathepsin L	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In an effort to uncover the cathepsin L expression in diverse pathological conditions in human testis , the immunohistochemical localization of cathepsin L was conducted in human testis under diverse male infertility condition including spermatogenic hypoplasia and testis cancer .
	manualset3
94442	7	400031	5	NULL	NULL	0	NULL	human testis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In an effort to uncover the cathepsin L expression in diverse pathological conditions in human testis , the immunohistochemical localization of cathepsin L was conducted in human testis under diverse male infertility condition including spermatogenic hypoplasia and testis cancer .
	manualset3
94443	8	400031	5	NULL	NULL	0	NULL	diverse male infertility condition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In an effort to uncover the cathepsin L expression in diverse pathological conditions in human testis , the immunohistochemical localization of cathepsin L was conducted in human testis under diverse male infertility condition including spermatogenic hypoplasia and testis cancer .
	manualset3
94446	9	400031	5	NULL	NULL	0	NULL	spermatogenic hypoplasia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In an effort to uncover the cathepsin L expression in diverse pathological conditions in human testis , the immunohistochemical localization of cathepsin L was conducted in human testis under diverse male infertility condition including spermatogenic hypoplasia and testis cancer .
	manualset3
94447	10	400031	5	NULL	NULL	0	NULL	testis cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In an effort to uncover the cathepsin L expression in diverse pathological conditions in human testis , the immunohistochemical localization of cathepsin L was conducted in human testis under diverse male infertility condition including spermatogenic hypoplasia and testis cancer .
	manualset3
94454	1	400032	5	NULL	NULL	0	NULL	initial study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In an initial study involving 31 subjects , angulations measured from dorsoplantar and lateral radiographs were compared with the corresponding Foot Posture Index criteria using Spearman 's rho and the generalized linear model of analysis of variance .
	manualset3
94455	2	400032	5	NULL	NULL	0	NULL	31 subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In an initial study involving 31 subjects , angulations measured from dorsoplantar and lateral radiographs were compared with the corresponding Foot Posture Index criteria using Spearman 's rho and the generalized linear model of analysis of variance .
	manualset3
94459	3	400032	5	NULL	NULL	0	NULL	angulations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In an initial study involving 31 subjects , angulations measured from dorsoplantar and lateral radiographs were compared with the corresponding Foot Posture Index criteria using Spearman 's rho and the generalized linear model of analysis of variance .
	manualset3
94460	4	400032	5	NULL	NULL	0	NULL	dorsoplantar and lateral radiographs	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In an initial study involving 31 subjects , angulations measured from dorsoplantar and lateral radiographs were compared with the corresponding Foot Posture Index criteria using Spearman 's rho and the generalized linear model of analysis of variance .
	manualset3
94502	5	400032	5	NULL	NULL	0	NULL	Spearman 's rho	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In an initial study involving 31 subjects , angulations measured from dorsoplantar and lateral radiographs were compared with the corresponding Foot Posture Index criteria using Spearman 's rho and the generalized linear model of analysis of variance .
	manualset3
94503	6	400032	5	NULL	NULL	0	NULL	generalized linear model of analysis of variance	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In an initial study involving 31 subjects , angulations measured from dorsoplantar and lateral radiographs were compared with the corresponding Foot Posture Index criteria using Spearman 's rho and the generalized linear model of analysis of variance .
	manualset3
94504	1	400033	5	NULL	NULL	0	NULL	anesthetized dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In anesthetized dogs , CL 115 , 347 injected intra-arterially ( 0.5-10 micrograms ) into the vascular bed being studied increased blood flow to femoral , carotid , coronary , superior mesenteric , and renal vascular beds .
	manualset3
94505	2	400033	5	NULL	NULL	0	NULL	CL 115 , 347	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In anesthetized dogs , CL 115 , 347 injected intra-arterially ( 0.5-10 micrograms ) into the vascular bed being studied increased blood flow to femoral , carotid , coronary , superior mesenteric , and renal vascular beds .
	manualset3
94506	3	400033	5	NULL	NULL	0	NULL	0.5-10 micrograms	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In anesthetized dogs , CL 115 , 347 injected intra-arterially ( 0.5-10 micrograms ) into the vascular bed being studied increased blood flow to femoral , carotid , coronary , superior mesenteric , and renal vascular beds .
	manualset3
94507	4	400033	5	NULL	NULL	0	NULL	vascular bed	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In anesthetized dogs , CL 115 , 347 injected intra-arterially ( 0.5-10 micrograms ) into the vascular bed being studied increased blood flow to femoral , carotid , coronary , superior mesenteric , and renal vascular beds .
	manualset3
94508	5	400033	5	NULL	NULL	0	NULL	blood flow	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In anesthetized dogs , CL 115 , 347 injected intra-arterially ( 0.5-10 micrograms ) into the vascular bed being studied increased blood flow to femoral , carotid , coronary , superior mesenteric , and renal vascular beds .
	manualset3
94509	6	400033	5	NULL	NULL	0	NULL	femoral vascular bed	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In anesthetized dogs , CL 115 , 347 injected intra-arterially ( 0.5-10 micrograms ) into the vascular bed being studied increased blood flow to femoral , carotid , coronary , superior mesenteric , and renal vascular beds .
	manualset3
94510	7	400033	5	NULL	NULL	0	NULL	carotid vascular bed	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In anesthetized dogs , CL 115 , 347 injected intra-arterially ( 0.5-10 micrograms ) into the vascular bed being studied increased blood flow to femoral , carotid , coronary , superior mesenteric , and renal vascular beds .
	manualset3
94511	8	400033	5	NULL	NULL	0	NULL	coronary vascular bed	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In anesthetized dogs , CL 115 , 347 injected intra-arterially ( 0.5-10 micrograms ) into the vascular bed being studied increased blood flow to femoral , carotid , coronary , superior mesenteric , and renal vascular beds .
	manualset3
94512	9	400033	5	NULL	NULL	0	NULL	superior mesenteric vascular bed	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In anesthetized dogs , CL 115 , 347 injected intra-arterially ( 0.5-10 micrograms ) into the vascular bed being studied increased blood flow to femoral , carotid , coronary , superior mesenteric , and renal vascular beds .
	manualset3
94513	10	400033	5	NULL	NULL	0	NULL	renal vascular beds	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In anesthetized dogs , CL 115 , 347 injected intra-arterially ( 0.5-10 micrograms ) into the vascular bed being studied increased blood flow to femoral , carotid , coronary , superior mesenteric , and renal vascular beds .
	manualset3
94514	1	400034	5	NULL	NULL	0	NULL	Vascular action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Vascular action of aldosterone ) .
	manualset3
94515	2	400034	5	NULL	NULL	0	NULL	aldosterone	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	( Vascular action of aldosterone ) .
	manualset3
94516	1	400035	5	NULL	NULL	0	NULL	animal models	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In animal models , a single dose of 17-AAG was sufficient to induce degradation of mutant EGFR and inhibit downstream signaling .
	manualset3
94517	2	400035	5	NULL	NULL	0	NULL	single dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In animal models , a single dose of 17-AAG was sufficient to induce degradation of mutant EGFR and inhibit downstream signaling .
	manualset3
94518	3	400035	5	NULL	NULL	0	NULL	17-AAG	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In animal models , a single dose of 17-AAG was sufficient to induce degradation of mutant EGFR and inhibit downstream signaling .
	manualset3
94519	4	400035	5	NULL	NULL	0	NULL	degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In animal models , a single dose of 17-AAG was sufficient to induce degradation of mutant EGFR and inhibit downstream signaling .
	manualset3
94520	5	400035	5	NULL	NULL	0	NULL	mutant EGFR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In animal models , a single dose of 17-AAG was sufficient to induce degradation of mutant EGFR and inhibit downstream signaling .
	manualset3
94521	6	400035	5	NULL	NULL	0	NULL	downstream signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In animal models , a single dose of 17-AAG was sufficient to induce degradation of mutant EGFR and inhibit downstream signaling .
	manualset3
94522	1	400036	5	NULL	NULL	0	NULL	 animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In animals orally intoxicated to verapamil , an intravenous injection of the liposomal antidote rapidly attenuated the reduction in blood pressure .
	manualset3
94523	2	400036	5	NULL	NULL	0	NULL	verapamil	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In animals orally intoxicated to verapamil , an intravenous injection of the liposomal antidote rapidly attenuated the reduction in blood pressure .
	manualset3
94524	3	400036	5	NULL	NULL	0	NULL	intravenous injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In animals orally intoxicated to verapamil , an intravenous injection of the liposomal antidote rapidly attenuated the reduction in blood pressure .
	manualset3
94525	4	400036	5	NULL	NULL	0	NULL	liposomal antidote	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In animals orally intoxicated to verapamil , an intravenous injection of the liposomal antidote rapidly attenuated the reduction in blood pressure .
	manualset3
94526	5	400036	5	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In animals orally intoxicated to verapamil , an intravenous injection of the liposomal antidote rapidly attenuated the reduction in blood pressure .
	manualset3
94527	6	400036	5	NULL	NULL	0	NULL	blood pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In animals orally intoxicated to verapamil , an intravenous injection of the liposomal antidote rapidly attenuated the reduction in blood pressure .
	manualset3
94528	1	400037	5	NULL	NULL	0	NULL	series of experiments 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In another series of experiments , uptake values for various anions as a percent of equilibrium ( I/E x 100 ) were : SCN - , 84.9 + / - 10.9 ; NO3 , 49.9 + / - 11.0 ; SO4 ( 2 - ) , 27.3 + / - 4.4 ; F - , 68.5 + / - 18.3 ; Cl - , 164.1 + / - 44.6 ; Br - , 150.6 + / - 30.2 ; I - , 56.7 + / - 13.5 .
	manualset3
94529	2	400037	5	NULL	NULL	0	NULL	uptake values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In another series of experiments , uptake values for various anions as a percent of equilibrium ( I/E x 100 ) were : SCN - , 84.9 + / - 10.9 ; NO3 , 49.9 + / - 11.0 ; SO4 ( 2 - ) , 27.3 + / - 4.4 ; F - , 68.5 + / - 18.3 ; Cl - , 164.1 + / - 44.6 ; Br - , 150.6 + / - 30.2 ; I - , 56.7 + / - 13.5 .
	manualset3
94530	3	400037	5	NULL	NULL	0	NULL	various anions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In another series of experiments , uptake values for various anions as a percent of equilibrium ( I/E x 100 ) were : SCN - , 84.9 + / - 10.9 ; NO3 , 49.9 + / - 11.0 ; SO4 ( 2 - ) , 27.3 + / - 4.4 ; F - , 68.5 + / - 18.3 ; Cl - , 164.1 + / - 44.6 ; Br - , 150.6 + / - 30.2 ; I - , 56.7 + / - 13.5 .
	manualset3
94531	4	400037	5	NULL	NULL	0	NULL	percent of equilibrium	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In another series of experiments , uptake values for various anions as a percent of equilibrium ( I/E x 100 ) were : SCN - , 84.9 + / - 10.9 ; NO3 , 49.9 + / - 11.0 ; SO4 ( 2 - ) , 27.3 + / - 4.4 ; F - , 68.5 + / - 18.3 ; Cl - , 164.1 + / - 44.6 ; Br - , 150.6 + / - 30.2 ; I - , 56.7 + / - 13.5 .
	manualset3
94532	5	400037	5	NULL	NULL	0	NULL	( I/E x 100 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In another series of experiments , uptake values for various anions as a percent of equilibrium ( I/E x 100 ) were : SCN - , 84.9 + / - 10.9 ; NO3 , 49.9 + / - 11.0 ; SO4 ( 2 - ) , 27.3 + / - 4.4 ; F - , 68.5 + / - 18.3 ; Cl - , 164.1 + / - 44.6 ; Br - , 150.6 + / - 30.2 ; I - , 56.7 + / - 13.5 .
	manualset3
94533	6	400037	5	NULL	NULL	0	NULL	SCN - , 84.9 + / - 10.9	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In another series of experiments , uptake values for various anions as a percent of equilibrium ( I/E x 100 ) were : SCN - , 84.9 + / - 10.9 ; NO3 , 49.9 + / - 11.0 ; SO4 ( 2 - ) , 27.3 + / - 4.4 ; F - , 68.5 + / - 18.3 ; Cl - , 164.1 + / - 44.6 ; Br - , 150.6 + / - 30.2 ; I - , 56.7 + / - 13.5 .
	manualset3
94534	7	400037	5	NULL	NULL	0	NULL	NO3 , 49.9 + / - 11.0	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In another series of experiments , uptake values for various anions as a percent of equilibrium ( I/E x 100 ) were : SCN - , 84.9 + / - 10.9 ; NO3 , 49.9 + / - 11.0 ; SO4 ( 2 - ) , 27.3 + / - 4.4 ; F - , 68.5 + / - 18.3 ; Cl - , 164.1 + / - 44.6 ; Br - , 150.6 + / - 30.2 ; I - , 56.7 + / - 13.5 .
	manualset3
94535	8	400037	5	NULL	NULL	0	NULL	SO4 ( 2 - ) , 27.3 + / - 4.4	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In another series of experiments , uptake values for various anions as a percent of equilibrium ( I/E x 100 ) were : SCN - , 84.9 + / - 10.9 ; NO3 , 49.9 + / - 11.0 ; SO4 ( 2 - ) , 27.3 + / - 4.4 ; F - , 68.5 + / - 18.3 ; Cl - , 164.1 + / - 44.6 ; Br - , 150.6 + / - 30.2 ; I - , 56.7 + / - 13.5 .
	manualset3
94536	9	400037	5	NULL	NULL	0	NULL	F - , 68.5 + / - 18.3	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In another series of experiments , uptake values for various anions as a percent of equilibrium ( I/E x 100 ) were : SCN - , 84.9 + / - 10.9 ; NO3 , 49.9 + / - 11.0 ; SO4 ( 2 - ) , 27.3 + / - 4.4 ; F - , 68.5 + / - 18.3 ; Cl - , 164.1 + / - 44.6 ; Br - , 150.6 + / - 30.2 ; I - , 56.7 + / - 13.5 .
	manualset3
94537	10	400037	5	NULL	NULL	0	NULL	Cl - , 164.1 + / - 44.6	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In another series of experiments , uptake values for various anions as a percent of equilibrium ( I/E x 100 ) were : SCN - , 84.9 + / - 10.9 ; NO3 , 49.9 + / - 11.0 ; SO4 ( 2 - ) , 27.3 + / - 4.4 ; F - , 68.5 + / - 18.3 ; Cl - , 164.1 + / - 44.6 ; Br - , 150.6 + / - 30.2 ; I - , 56.7 + / - 13.5 .
	manualset3
94538	11	400037	5	NULL	NULL	0	NULL	Br - , 150.6 + / - 30.2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In another series of experiments , uptake values for various anions as a percent of equilibrium ( I/E x 100 ) were : SCN - , 84.9 + / - 10.9 ; NO3 , 49.9 + / - 11.0 ; SO4 ( 2 - ) , 27.3 + / - 4.4 ; F - , 68.5 + / - 18.3 ; Cl - , 164.1 + / - 44.6 ; Br - , 150.6 + / - 30.2 ; I - , 56.7 + / - 13.5 .
	manualset3
94539	12	400037	5	NULL	NULL	0	NULL	I - , 56.7 + / - 13.5	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In another series of experiments , uptake values for various anions as a percent of equilibrium ( I/E x 100 ) were : SCN - , 84.9 + / - 10.9 ; NO3 , 49.9 + / - 11.0 ; SO4 ( 2 - ) , 27.3 + / - 4.4 ; F - , 68.5 + / - 18.3 ; Cl - , 164.1 + / - 44.6 ; Br - , 150.6 + / - 30.2 ; I - , 56.7 + / - 13.5 .
	manualset3
94540	1	400038	5	NULL	NULL	0	NULL	antidiuresis rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In antidiuresis rats the extract significantly increased reabsorption of water by the collecting duct and in water diuresis animals the extract significantly increased free water clearance .
	manualset3
95044	2	400038	5	NULL	NULL	0	NULL	extract	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In antidiuresis rats the extract significantly increased reabsorption of water by the collecting duct and in water diuresis animals the extract significantly increased free water clearance .
	manualset3
95045	3	400038	5	NULL	NULL	0	NULL	reabsorption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In antidiuresis rats the extract significantly increased reabsorption of water by the collecting duct and in water diuresis animals the extract significantly increased free water clearance .
	manualset3
95046	4	400038	5	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In antidiuresis rats the extract significantly increased reabsorption of water by the collecting duct and in water diuresis animals the extract significantly increased free water clearance .
	manualset3
95047	5	400038	5	NULL	NULL	0	NULL	collecting duct	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In antidiuresis rats the extract significantly increased reabsorption of water by the collecting duct and in water diuresis animals the extract significantly increased free water clearance .
	manualset3
95048	6	400038	5	NULL	NULL	0	NULL	water diuresis animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In antidiuresis rats the extract significantly increased reabsorption of water by the collecting duct and in water diuresis animals the extract significantly increased free water clearance .
	manualset3
95049	7	400038	5	NULL	NULL	0	NULL	extract 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In antidiuresis rats the extract significantly increased reabsorption of water by the collecting duct and in water diuresis animals the extract significantly increased free water clearance .
	manualset3
95050	8	400038	5	NULL	NULL	NULL	NULL	free water clearance 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In antidiuresis rats the extract significantly increased reabsorption of water by the collecting duct and in water diuresis animals the extract significantly increased free water clearance .
	manualset3
95051	1	400039	5	NULL	NULL	0	NULL	urinary metabolite profile	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In any case , the urinary metabolite profile of antipyrine can be used to study changes in the activity of different cytochromes in drug metabolism studies .
	manualset3
95052	2	400039	5	NULL	NULL	0	NULL	antipyrine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In any case , the urinary metabolite profile of antipyrine can be used to study changes in the activity of different cytochromes in drug metabolism studies .
	manualset3
95053	3	400039	5	NULL	NULL	0	NULL	activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In any case , the urinary metabolite profile of antipyrine can be used to study changes in the activity of different cytochromes in drug metabolism studies .
	manualset3
95054	4	400039	5	NULL	NULL	0	NULL	cytochromes	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In any case , the urinary metabolite profile of antipyrine can be used to study changes in the activity of different cytochromes in drug metabolism studies .
	manualset3
95055	5	400039	5	NULL	NULL	0	NULL	drug metabolism studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In any case , the urinary metabolite profile of antipyrine can be used to study changes in the activity of different cytochromes in drug metabolism studies .
	manualset3
95056	1	400040	5	NULL	NULL	0	NULL	aqueous medium 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In aqueous medium of pH 2.09 , there are about 2.2 x 10 ( 3 ) Cap molecules covalently binding to the surface of a 10-nm diameter gold nanoparticle through the thiol functional group of Cap , and thus forms a core-shell assembly of ( ( Au ) ( 31000 ) ) @ ( ( Cap ) ( 2200 ) ) , displaying strong enhanced PRLS signals in the PRA region of gold colloid .
	manualset3
95057	2	400040	5	NULL	NULL	0	NULL	pH 2.09 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In aqueous medium of pH 2.09 , there are about 2.2 x 10 ( 3 ) Cap molecules covalently binding to the surface of a 10-nm diameter gold nanoparticle through the thiol functional group of Cap , and thus forms a core-shell assembly of ( ( Au ) ( 31000 ) ) @ ( ( Cap ) ( 2200 ) ) , displaying strong enhanced PRLS signals in the PRA region of gold colloid .
	manualset3
95058	3	400040	5	NULL	NULL	0	NULL	2.2 x 10 ( 3 ) Cap molecules	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In aqueous medium of pH 2.09 , there are about 2.2 x 10 ( 3 ) Cap molecules covalently binding to the surface of a 10-nm diameter gold nanoparticle through the thiol functional group of Cap , and thus forms a core-shell assembly of ( ( Au ) ( 31000 ) ) @ ( ( Cap ) ( 2200 ) ) , displaying strong enhanced PRLS signals in the PRA region of gold colloid .
	manualset3
95059	4	400040	5	NULL	NULL	0	NULL	10-nm diameter gold nanoparticle	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In aqueous medium of pH 2.09 , there are about 2.2 x 10 ( 3 ) Cap molecules covalently binding to the surface of a 10-nm diameter gold nanoparticle through the thiol functional group of Cap , and thus forms a core-shell assembly of ( ( Au ) ( 31000 ) ) @ ( ( Cap ) ( 2200 ) ) , displaying strong enhanced PRLS signals in the PRA region of gold colloid .
	manualset3
95060	5	400040	5	NULL	NULL	0	NULL	thiol functional group	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In aqueous medium of pH 2.09 , there are about 2.2 x 10 ( 3 ) Cap molecules covalently binding to the surface of a 10-nm diameter gold nanoparticle through the thiol functional group of Cap , and thus forms a core-shell assembly of ( ( Au ) ( 31000 ) ) @ ( ( Cap ) ( 2200 ) ) , displaying strong enhanced PRLS signals in the PRA region of gold colloid .
	manualset3
95061	6	400040	5	NULL	NULL	0	NULL	Cap 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In aqueous medium of pH 2.09 , there are about 2.2 x 10 ( 3 ) Cap molecules covalently binding to the surface of a 10-nm diameter gold nanoparticle through the thiol functional group of Cap , and thus forms a core-shell assembly of ( ( Au ) ( 31000 ) ) @ ( ( Cap ) ( 2200 ) ) , displaying strong enhanced PRLS signals in the PRA region of gold colloid .
	manualset3
95062	7	400040	5	NULL	NULL	0	NULL	core-shell assembly	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In aqueous medium of pH 2.09 , there are about 2.2 x 10 ( 3 ) Cap molecules covalently binding to the surface of a 10-nm diameter gold nanoparticle through the thiol functional group of Cap , and thus forms a core-shell assembly of ( ( Au ) ( 31000 ) ) @ ( ( Cap ) ( 2200 ) ) , displaying strong enhanced PRLS signals in the PRA region of gold colloid .
	manualset3
95063	8	400040	5	NULL	NULL	0	NULL	( ( Au ) ( 31000 ) ) @ ( ( Cap ) ( 2200 ) )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In aqueous medium of pH 2.09 , there are about 2.2 x 10 ( 3 ) Cap molecules covalently binding to the surface of a 10-nm diameter gold nanoparticle through the thiol functional group of Cap , and thus forms a core-shell assembly of ( ( Au ) ( 31000 ) ) @ ( ( Cap ) ( 2200 ) ) , displaying strong enhanced PRLS signals in the PRA region of gold colloid .
	manualset3
95064	9	400040	5	NULL	NULL	0	NULL	strong enhanced PRLS signals	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In aqueous medium of pH 2.09 , there are about 2.2 x 10 ( 3 ) Cap molecules covalently binding to the surface of a 10-nm diameter gold nanoparticle through the thiol functional group of Cap , and thus forms a core-shell assembly of ( ( Au ) ( 31000 ) ) @ ( ( Cap ) ( 2200 ) ) , displaying strong enhanced PRLS signals in the PRA region of gold colloid .
	manualset3
95065	10	400040	5	NULL	NULL	0	NULL	PRA region of gold colloid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In aqueous medium of pH 2.09 , there are about 2.2 x 10 ( 3 ) Cap molecules covalently binding to the surface of a 10-nm diameter gold nanoparticle through the thiol functional group of Cap , and thus forms a core-shell assembly of ( ( Au ) ( 31000 ) ) @ ( ( Cap ) ( 2200 ) ) , displaying strong enhanced PRLS signals in the PRA region of gold colloid .
	manualset3
95066	1	400041	5	NULL	NULL	0	NULL	areas	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In areas with PMN in idiopathic autoimmune CALD ( IA-CALD , n = 15 ) OKT8 + and OKM + lymphocytes and IgG plasma cells were present , whereas in hepatitis B-CALD ( HB-CALD , n = 12 ) almost exclusively OKT8 + cells were found .
	manualset3
95067	2	400041	5	NULL	NULL	0	NULL	PMN	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In areas with PMN in idiopathic autoimmune CALD ( IA-CALD , n = 15 ) OKT8 + and OKM + lymphocytes and IgG plasma cells were present , whereas in hepatitis B-CALD ( HB-CALD , n = 12 ) almost exclusively OKT8 + cells were found .
	manualset3
95068	3	400041	5	NULL	NULL	NULL	NULL	idiopathic autoimmune CALD	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In areas with PMN in idiopathic autoimmune CALD ( IA-CALD , n = 15 ) OKT8 + and OKM + lymphocytes and IgG plasma cells were present , whereas in hepatitis B-CALD ( HB-CALD , n = 12 ) almost exclusively OKT8 + cells were found .
	manualset3
95069	6	400041	5	NULL	NULL	NULL	NULL	IgG plasma cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In areas with PMN in idiopathic autoimmune CALD ( IA-CALD , n = 15 ) OKT8 + and OKM + lymphocytes and IgG plasma cells were present , whereas in hepatitis B-CALD ( HB-CALD , n = 12 ) almost exclusively OKT8 + cells were found .
	manualset3
95070	4	400041	5	NULL	NULL	0	NULL	( IA-CALD , n = 15 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In areas with PMN in idiopathic autoimmune CALD ( IA-CALD , n = 15 ) OKT8 + and OKM + lymphocytes and IgG plasma cells were present , whereas in hepatitis B-CALD ( HB-CALD , n = 12 ) almost exclusively OKT8 + cells were found .
	manualset3
95071	5	400041	5	NULL	NULL	0	NULL	OKT8 + and OKM + lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In areas with PMN in idiopathic autoimmune CALD ( IA-CALD , n = 15 ) OKT8 + and OKM + lymphocytes and IgG plasma cells were present , whereas in hepatitis B-CALD ( HB-CALD , n = 12 ) almost exclusively OKT8 + cells were found .
	manualset3
95072	7	400041	5	NULL	NULL	0	NULL	hepatitis B-CALD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In areas with PMN in idiopathic autoimmune CALD ( IA-CALD , n = 15 ) OKT8 + and OKM + lymphocytes and IgG plasma cells were present , whereas in hepatitis B-CALD ( HB-CALD , n = 12 ) almost exclusively OKT8 + cells were found .
	manualset3
95073	8	400041	5	NULL	NULL	0	NULL	( HB-CALD , n = 12 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In areas with PMN in idiopathic autoimmune CALD ( IA-CALD , n = 15 ) OKT8 + and OKM + lymphocytes and IgG plasma cells were present , whereas in hepatitis B-CALD ( HB-CALD , n = 12 ) almost exclusively OKT8 + cells were found .
	manualset3
95074	9	400041	5	NULL	NULL	0	NULL	OKT8 + cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In areas with PMN in idiopathic autoimmune CALD ( IA-CALD , n = 15 ) OKT8 + and OKM + lymphocytes and IgG plasma cells were present , whereas in hepatitis B-CALD ( HB-CALD , n = 12 ) almost exclusively OKT8 + cells were found .
	manualset3
95075	1	400042	5	NULL	NULL	0	NULL	axial muscles	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In axial muscles , slow-twitch fibers and fast-twitch fibers composed predominantly of type IIB were distributed dispersively .
	manualset3
95076	2	400042	5	NULL	NULL	0	NULL	slow-twitch fibers	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In axial muscles , slow-twitch fibers and fast-twitch fibers composed predominantly of type IIB were distributed dispersively .
	manualset3
95077	3	400042	5	NULL	NULL	0	NULL	slow-twitch fibers	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In axial muscles , slow-twitch fibers and fast-twitch fibers composed predominantly of type IIB were distributed dispersively .
	manualset3
95078	4	400042	5	NULL	NULL	0	NULL	fast-twitch fibers	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In axial muscles , slow-twitch fibers and fast-twitch fibers composed predominantly of type IIB were distributed dispersively .
	manualset3
95079	5	400042	5	NULL	NULL	0	NULL	type IIB	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In axial muscles , slow-twitch fibers and fast-twitch fibers composed predominantly of type IIB were distributed dispersively .
	manualset3
95080	1	400043	5	NULL	NULL	0	NULL	Vascular changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Vascular changes of bone marrow in granulocytic myeloses ) .
	manualset3
95081	2	400043	5	NULL	NULL	0	NULL	bone marrow	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Vascular changes of bone marrow in granulocytic myeloses ) .
	manualset3
95082	3	400043	5	NULL	NULL	0	NULL	granulocytic myeloses	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Vascular changes of bone marrow in granulocytic myeloses ) .
	manualset3
95083	1	400044	5	NULL	NULL	NULL	NULL	axin mutants	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In axin mutants , Arm is localized to the nuclei .
	manualset3
95084	2	400044	5	NULL	NULL	0	NULL	Arm	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In axin mutants , Arm is localized to the nuclei .
	manualset3
95085	3	400044	5	NULL	NULL	0	NULL	nuclei	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In axin mutants , Arm is localized to the nuclei .
	manualset3
95086	1	400045	5	NULL	NULL	0	NULL	barium enemas	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In barium enemas it is recommended to give the drug at the beginning of the examination .
	manualset3
95087	2	400045	5	NULL	NULL	0	NULL	drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In barium enemas it is recommended to give the drug at the beginning of the examination .
	manualset3
95088	3	400045	5	NULL	NULL	0	NULL	examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In barium enemas it is recommended to give the drug at the beginning of the examination .
	manualset3
95089	1	400046	5	NULL	NULL	NULL	NULL	biodistribution	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In biodistribution and dynamic micro-MRI studies , significantly less renal accumulation of G7D - ( 1B4M-Gd ) ( 512 ) , G8D - ( 1B4M-Gd ) ( 1024 ) , and G9D - ( 1B4M-Gd ) ( 2048 ) was shown compared to G6D - ( 1B4M-Gd ) ( 256 ) ( P & lt ; 0.01 ) .
	manualset3
95090	2	400046	5	NULL	NULL	0	NULL	dynamic micro-MRI studies 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In biodistribution and dynamic micro-MRI studies , significantly less renal accumulation of G7D - ( 1B4M-Gd ) ( 512 ) , G8D - ( 1B4M-Gd ) ( 1024 ) , and G9D - ( 1B4M-Gd ) ( 2048 ) was shown compared to G6D - ( 1B4M-Gd ) ( 256 ) ( P & lt ; 0.01 ) .
	manualset3
95091	3	400046	5	NULL	NULL	0	NULL	significantly less renal accumulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In biodistribution and dynamic micro-MRI studies , significantly less renal accumulation of G7D - ( 1B4M-Gd ) ( 512 ) , G8D - ( 1B4M-Gd ) ( 1024 ) , and G9D - ( 1B4M-Gd ) ( 2048 ) was shown compared to G6D - ( 1B4M-Gd ) ( 256 ) ( P & lt ; 0.01 ) .
	manualset3
95092	4	400046	5	NULL	NULL	0	NULL	G7D - ( 1B4M-Gd ) ( 512 )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In biodistribution and dynamic micro-MRI studies , significantly less renal accumulation of G7D - ( 1B4M-Gd ) ( 512 ) , G8D - ( 1B4M-Gd ) ( 1024 ) , and G9D - ( 1B4M-Gd ) ( 2048 ) was shown compared to G6D - ( 1B4M-Gd ) ( 256 ) ( P & lt ; 0.01 ) .
	manualset3
95093	5	400046	5	NULL	NULL	0	NULL	G8D - ( 1B4M-Gd ) ( 1024 )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In biodistribution and dynamic micro-MRI studies , significantly less renal accumulation of G7D - ( 1B4M-Gd ) ( 512 ) , G8D - ( 1B4M-Gd ) ( 1024 ) , and G9D - ( 1B4M-Gd ) ( 2048 ) was shown compared to G6D - ( 1B4M-Gd ) ( 256 ) ( P & lt ; 0.01 ) .
	manualset3
95094	6	400046	5	NULL	NULL	0	NULL	G8D - ( 1B4M-Gd ) ( 1024 )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In biodistribution and dynamic micro-MRI studies , significantly less renal accumulation of G7D - ( 1B4M-Gd ) ( 512 ) , G8D - ( 1B4M-Gd ) ( 1024 ) , and G9D - ( 1B4M-Gd ) ( 2048 ) was shown compared to G6D - ( 1B4M-Gd ) ( 256 ) ( P & lt ; 0.01 ) .
	manualset3
95095	7	400046	5	NULL	NULL	0	NULL	G6D - ( 1B4M-Gd ) ( 256 )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In biodistribution and dynamic micro-MRI studies , significantly less renal accumulation of G7D - ( 1B4M-Gd ) ( 512 ) , G8D - ( 1B4M-Gd ) ( 1024 ) , and G9D - ( 1B4M-Gd ) ( 2048 ) was shown compared to G6D - ( 1B4M-Gd ) ( 256 ) ( P & lt ; 0.01 ) .
	manualset3
95096	8	400046	5	NULL	NULL	0	NULL	( P & lt ; 0.01 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In biodistribution and dynamic micro-MRI studies , significantly less renal accumulation of G7D - ( 1B4M-Gd ) ( 512 ) , G8D - ( 1B4M-Gd ) ( 1024 ) , and G9D - ( 1B4M-Gd ) ( 2048 ) was shown compared to G6D - ( 1B4M-Gd ) ( 256 ) ( P & lt ; 0.01 ) .
	manualset3
95097	1	400047	5	NULL	NULL	NULL	NULL	biological systems	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In biological systems , complex molecules interact with specificity and rapidity .
	manualset3
95098	2	400047	5	NULL	NULL	0	NULL	complex molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In biological systems , complex molecules interact with specificity and rapidity .
	manualset3
95099	1	400048	5	NULL	NULL	0	NULL	biologically active peptide analogs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In biologically active peptide analogs , the aza-substitution has led to enhanced activity and selectivity as well as improved properties , such as prolonged duration of action and metabolic stability .
	manualset3
95100	2	400048	5	NULL	NULL	0	NULL	aza-substitution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In biologically active peptide analogs , the aza-substitution has led to enhanced activity and selectivity as well as improved properties , such as prolonged duration of action and metabolic stability .
	manualset3
95101	3	400048	5	NULL	NULL	0	NULL	enhanced activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In biologically active peptide analogs , the aza-substitution has led to enhanced activity and selectivity as well as improved properties , such as prolonged duration of action and metabolic stability .
	manualset3
95102	4	400048	5	NULL	NULL	0	NULL	selectivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In biologically active peptide analogs , the aza-substitution has led to enhanced activity and selectivity as well as improved properties , such as prolonged duration of action and metabolic stability .
	manualset3
95103	5	400048	5	NULL	NULL	0	NULL	improved properties 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In biologically active peptide analogs , the aza-substitution has led to enhanced activity and selectivity as well as improved properties , such as prolonged duration of action and metabolic stability .
	manualset3
95104	6	400048	5	NULL	NULL	0	NULL	prolonged duration of action	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In biologically active peptide analogs , the aza-substitution has led to enhanced activity and selectivity as well as improved properties , such as prolonged duration of action and metabolic stability .
	manualset3
95105	7	400048	5	NULL	NULL	0	NULL	metabolic stability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In biologically active peptide analogs , the aza-substitution has led to enhanced activity and selectivity as well as improved properties , such as prolonged duration of action and metabolic stability .
	manualset3
95106	1	400049	5	NULL	NULL	0	NULL	birds	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In birds fed rations containing only 10 mg of FB1/kg , bile duct hyperplasia with fibrosis and a mononuclear infiltrate accompanied by trabecular derangement were observed .
	manualset3
95107	2	400049	5	NULL	NULL	0	NULL	rations	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	In birds fed rations containing only 10 mg of FB1/kg , bile duct hyperplasia with fibrosis and a mononuclear infiltrate accompanied by trabecular derangement were observed .
	manualset3
95108	3	400049	5	NULL	NULL	0	NULL	10 mg of FB1/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In birds fed rations containing only 10 mg of FB1/kg , bile duct hyperplasia with fibrosis and a mononuclear infiltrate accompanied by trabecular derangement were observed .
	manualset3
95109	4	400049	5	NULL	NULL	0	NULL	bile duct hyperplasia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In birds fed rations containing only 10 mg of FB1/kg , bile duct hyperplasia with fibrosis and a mononuclear infiltrate accompanied by trabecular derangement were observed .
	manualset3
95110	5	400049	5	NULL	NULL	0	NULL	fibrosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In birds fed rations containing only 10 mg of FB1/kg , bile duct hyperplasia with fibrosis and a mononuclear infiltrate accompanied by trabecular derangement were observed .
	manualset3
95111	6	400049	5	NULL	NULL	0	NULL	mononuclear infiltrate accompanied by trabecular derangement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In birds fed rations containing only 10 mg of FB1/kg , bile duct hyperplasia with fibrosis and a mononuclear infiltrate accompanied by trabecular derangement were observed .
	manualset3
95112	1	400050	5	NULL	NULL	0	NULL	 primary and secondary MLC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In both primary and secondary MLC between responder spleen cells from non-transgenic ( B6 X SJL/J ) F1 mice and transgenic stimulator cells , CTL were generated that specifically lysed mouse L cell ( H-2k ) or human B cell targets expressing HLA-B27 , and this lysis thus appeared largely unrestricted by H-2 .
	manualset3
95113	2	400050	5	NULL	NULL	0	NULL	responder spleen cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In both primary and secondary MLC between responder spleen cells from non-transgenic ( B6 X SJL/J ) F1 mice and transgenic stimulator cells , CTL were generated that specifically lysed mouse L cell ( H-2k ) or human B cell targets expressing HLA-B27 , and this lysis thus appeared largely unrestricted by H-2 .
	manualset3
95114	3	400050	5	NULL	NULL	0	NULL	non-transgenic ( B6 X SJL/J ) F1 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In both primary and secondary MLC between responder spleen cells from non-transgenic ( B6 X SJL/J ) F1 mice and transgenic stimulator cells , CTL were generated that specifically lysed mouse L cell ( H-2k ) or human B cell targets expressing HLA-B27 , and this lysis thus appeared largely unrestricted by H-2 .
	manualset3
95115	4	400050	5	NULL	NULL	0	NULL	transgenic stimulator cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In both primary and secondary MLC between responder spleen cells from non-transgenic ( B6 X SJL/J ) F1 mice and transgenic stimulator cells , CTL were generated that specifically lysed mouse L cell ( H-2k ) or human B cell targets expressing HLA-B27 , and this lysis thus appeared largely unrestricted by H-2 .
	manualset3
95116	5	400050	5	NULL	NULL	NULL	NULL	CTL	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In both primary and secondary MLC between responder spleen cells from non-transgenic ( B6 X SJL/J ) F1 mice and transgenic stimulator cells , CTL were generated that specifically lysed mouse L cell ( H-2k ) or human B cell targets expressing HLA-B27 , and this lysis thus appeared largely unrestricted by H-2 .
	manualset3
95117	6	400050	5	NULL	NULL	0	NULL	mouse L cell ( H-2k )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In both primary and secondary MLC between responder spleen cells from non-transgenic ( B6 X SJL/J ) F1 mice and transgenic stimulator cells , CTL were generated that specifically lysed mouse L cell ( H-2k ) or human B cell targets expressing HLA-B27 , and this lysis thus appeared largely unrestricted by H-2 .
	manualset3
95118	7	400050	5	NULL	NULL	NULL	NULL	human B cell targets expressing HLA-B27	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In both primary and secondary MLC between responder spleen cells from non-transgenic ( B6 X SJL/J ) F1 mice and transgenic stimulator cells , CTL were generated that specifically lysed mouse L cell ( H-2k ) or human B cell targets expressing HLA-B27 , and this lysis thus appeared largely unrestricted by H-2 .
	manualset3
95120	8	400050	5	NULL	NULL	NULL	NULL	lysis	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In both primary and secondary MLC between responder spleen cells from non-transgenic ( B6 X SJL/J ) F1 mice and transgenic stimulator cells , CTL were generated that specifically lysed mouse L cell ( H-2k ) or human B cell targets expressing HLA-B27 , and this lysis thus appeared largely unrestricted by H-2 .
	manualset3
95121	9	400050	5	NULL	NULL	NULL	NULL	H-2	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In both primary and secondary MLC between responder spleen cells from non-transgenic ( B6 X SJL/J ) F1 mice and transgenic stimulator cells , CTL were generated that specifically lysed mouse L cell ( H-2k ) or human B cell targets expressing HLA-B27 , and this lysis thus appeared largely unrestricted by H-2 .
	manualset3
95131	1	400051	5	NULL	NULL	0	NULL	sham and PBD rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In both sham and PBD rats , feeding of a high-protein diet for 2 days induced phosphorylation of eukaryotic initiation factor 4E-binding protein 1 and 70-kDa ribosomal protein S6 kinase , indicating the activation of the initiation phase of translation for pancreatic protein synthesis .
	manualset3
95190	2	400051	5	NULL	NULL	0	NULL	 high-protein diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	In both sham and PBD rats , feeding of a high-protein diet for 2 days induced phosphorylation of eukaryotic initiation factor 4E-binding protein 1 and 70-kDa ribosomal protein S6 kinase , indicating the activation of the initiation phase of translation for pancreatic protein synthesis .
	manualset3
95195	3	400051	5	NULL	NULL	0	NULL	2 days	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In both sham and PBD rats , feeding of a high-protein diet for 2 days induced phosphorylation of eukaryotic initiation factor 4E-binding protein 1 and 70-kDa ribosomal protein S6 kinase , indicating the activation of the initiation phase of translation for pancreatic protein synthesis .
	manualset3
95196	4	400051	5	NULL	NULL	0	NULL	phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In both sham and PBD rats , feeding of a high-protein diet for 2 days induced phosphorylation of eukaryotic initiation factor 4E-binding protein 1 and 70-kDa ribosomal protein S6 kinase , indicating the activation of the initiation phase of translation for pancreatic protein synthesis .
	manualset3
95197	5	400051	5	NULL	NULL	0	NULL	eukaryotic initiation factor 4E-binding protein 1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In both sham and PBD rats , feeding of a high-protein diet for 2 days induced phosphorylation of eukaryotic initiation factor 4E-binding protein 1 and 70-kDa ribosomal protein S6 kinase , indicating the activation of the initiation phase of translation for pancreatic protein synthesis .
	manualset3
95206	6	400051	5	NULL	NULL	0	NULL	70-kDa ribosomal protein S6 kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In both sham and PBD rats , feeding of a high-protein diet for 2 days induced phosphorylation of eukaryotic initiation factor 4E-binding protein 1 and 70-kDa ribosomal protein S6 kinase , indicating the activation of the initiation phase of translation for pancreatic protein synthesis .
	manualset3
95207	7	400051	5	NULL	NULL	0	NULL	activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In both sham and PBD rats , feeding of a high-protein diet for 2 days induced phosphorylation of eukaryotic initiation factor 4E-binding protein 1 and 70-kDa ribosomal protein S6 kinase , indicating the activation of the initiation phase of translation for pancreatic protein synthesis .
	manualset3
95209	8	400051	5	NULL	NULL	0	NULL	initiation phase of translation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In both sham and PBD rats , feeding of a high-protein diet for 2 days induced phosphorylation of eukaryotic initiation factor 4E-binding protein 1 and 70-kDa ribosomal protein S6 kinase , indicating the activation of the initiation phase of translation for pancreatic protein synthesis .
	manualset3
95212	9	400051	5	NULL	NULL	0	NULL	pancreatic protein synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In both sham and PBD rats , feeding of a high-protein diet for 2 days induced phosphorylation of eukaryotic initiation factor 4E-binding protein 1 and 70-kDa ribosomal protein S6 kinase , indicating the activation of the initiation phase of translation for pancreatic protein synthesis .
	manualset3
95214	1	400052	5	NULL	NULL	NULL	NULL	normal fibers	AnatomicalPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In both normal fibers and fibers without tubules , measurements of input resistance and diameter were made at normal pH and at low pH when the chloride conductance was very small .
	manualset3
95215	2	400052	5	NULL	NULL	NULL	NULL	fibers without tubules	AnatomicalPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In both normal fibers and fibers without tubules , measurements of input resistance and diameter were made at normal pH and at low pH when the chloride conductance was very small .
	manualset3
95216	3	400052	5	NULL	NULL	0	NULL	measurements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In both normal fibers and fibers without tubules , measurements of input resistance and diameter were made at normal pH and at low pH when the chloride conductance was very small .
	manualset3
95217	4	400052	5	NULL	NULL	NULL	NULL	input resistance 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In both normal fibers and fibers without tubules , measurements of input resistance and diameter were made at normal pH and at low pH when the chloride conductance was very small .
	manualset3
95218	5	400052	5	NULL	NULL	0	NULL	diameter 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In both normal fibers and fibers without tubules , measurements of input resistance and diameter were made at normal pH and at low pH when the chloride conductance was very small .
	manualset3
95219	6	400052	5	NULL	NULL	0	NULL	normal pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In both normal fibers and fibers without tubules , measurements of input resistance and diameter were made at normal pH and at low pH when the chloride conductance was very small .
	manualset3
95220	7	400052	5	NULL	NULL	0	NULL	low pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In both normal fibers and fibers without tubules , measurements of input resistance and diameter were made at normal pH and at low pH when the chloride conductance was very small .
	manualset3
95221	8	400052	5	NULL	NULL	0	NULL	chloride conductance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In both normal fibers and fibers without tubules , measurements of input resistance and diameter were made at normal pH and at low pH when the chloride conductance was very small .
	manualset3
95222	1	400053	5	NULL	NULL	0	NULL	Antibiotic resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Antibiotic resistance and molecular typing of Listeria monocytogenes from foods in Shandong province from 2009 to 2010 ) .
	manualset3
95223	2	400053	5	NULL	NULL	0	NULL	molecular typing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Antibiotic resistance and molecular typing of Listeria monocytogenes from foods in Shandong province from 2009 to 2010 ) .
	manualset3
95224	3	400053	5	NULL	NULL	0	NULL	Listeria monocytogenes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Antibiotic resistance and molecular typing of Listeria monocytogenes from foods in Shandong province from 2009 to 2010 ) .
	manualset3
95225	4	400053	5	NULL	NULL	0	NULL	foods 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	( Antibiotic resistance and molecular typing of Listeria monocytogenes from foods in Shandong province from 2009 to 2010 ) .
	manualset3
95226	5	400053	5	NULL	NULL	0	NULL	Shandong province	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Antibiotic resistance and molecular typing of Listeria monocytogenes from foods in Shandong province from 2009 to 2010 ) .
	manualset3
95227	6	400053	5	NULL	NULL	0	NULL	from 2009 to 2010	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	( Antibiotic resistance and molecular typing of Listeria monocytogenes from foods in Shandong province from 2009 to 2010 ) .
	manualset3
95228	1	400054	5	NULL	NULL	0	NULL	Vasoconstrictors	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Vasoconstrictors added to dental local anesthetics ) .
	manualset3
95229	2	400054	5	NULL	NULL	0	NULL	dental local anesthetics	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Vasoconstrictors added to dental local anesthetics ) .
	manualset3
95230	1	400055	5	NULL	NULL	0	NULL	primary AP cell cultures 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In both primary AP cell cultures and the AP gland , in situ expression of TH was seen in lactotrophs , somatotrophs , corticotrophs , thyrotrophs , and gonadotrophs in the absence but not presence of doxycycline .
	manualset3
95231	2	400055	5	NULL	NULL	0	NULL	AP gland	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In both primary AP cell cultures and the AP gland , in situ expression of TH was seen in lactotrophs , somatotrophs , corticotrophs , thyrotrophs , and gonadotrophs in the absence but not presence of doxycycline .
	manualset3
95232	3	400055	5	NULL	NULL	0	NULL	in situ expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In both primary AP cell cultures and the AP gland , in situ expression of TH was seen in lactotrophs , somatotrophs , corticotrophs , thyrotrophs , and gonadotrophs in the absence but not presence of doxycycline .
	manualset3
95233	4	400055	5	NULL	NULL	0	NULL	TH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In both primary AP cell cultures and the AP gland , in situ expression of TH was seen in lactotrophs , somatotrophs , corticotrophs , thyrotrophs , and gonadotrophs in the absence but not presence of doxycycline .
	manualset3
95234	5	400055	5	NULL	NULL	NULL	NULL	lactotrophs	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In both primary AP cell cultures and the AP gland , in situ expression of TH was seen in lactotrophs , somatotrophs , corticotrophs , thyrotrophs , and gonadotrophs in the absence but not presence of doxycycline .
	manualset3
95235	6	400055	5	NULL	NULL	NULL	NULL	somatotrophs	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In both primary AP cell cultures and the AP gland , in situ expression of TH was seen in lactotrophs , somatotrophs , corticotrophs , thyrotrophs , and gonadotrophs in the absence but not presence of doxycycline .
	manualset3
95236	7	400055	5	NULL	NULL	0	NULL	corticotrophs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In both primary AP cell cultures and the AP gland , in situ expression of TH was seen in lactotrophs , somatotrophs , corticotrophs , thyrotrophs , and gonadotrophs in the absence but not presence of doxycycline .
	manualset3
95237	8	400055	5	NULL	NULL	0	NULL	thyrotrophs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In both primary AP cell cultures and the AP gland , in situ expression of TH was seen in lactotrophs , somatotrophs , corticotrophs , thyrotrophs , and gonadotrophs in the absence but not presence of doxycycline .
	manualset3
95238	9	400055	5	NULL	NULL	0	NULL	gonadotrophs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In both primary AP cell cultures and the AP gland , in situ expression of TH was seen in lactotrophs , somatotrophs , corticotrophs , thyrotrophs , and gonadotrophs in the absence but not presence of doxycycline .
	manualset3
95239	10	400055	5	NULL	NULL	0	NULL	doxycycline 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In both primary AP cell cultures and the AP gland , in situ expression of TH was seen in lactotrophs , somatotrophs , corticotrophs , thyrotrophs , and gonadotrophs in the absence but not presence of doxycycline .
	manualset3
95240	1	400056	5	NULL	NULL	NULL	NULL	study populations	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In both the study and control populations , Chlamydia antigen was more prevalent among younger women and non-contraceptive users .
	manualset3
95241	2	400056	5	NULL	NULL	0	NULL	control populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In both the study and control populations , Chlamydia antigen was more prevalent among younger women and non-contraceptive users .
	manualset3
95242	3	400056	5	NULL	NULL	0	NULL	Chlamydia antigen	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In both the study and control populations , Chlamydia antigen was more prevalent among younger women and non-contraceptive users .
	manualset3
95243	4	400056	5	NULL	NULL	0	NULL	younger women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In both the study and control populations , Chlamydia antigen was more prevalent among younger women and non-contraceptive users .
	manualset3
95244	5	400056	5	NULL	NULL	0	NULL	non-contraceptive users	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In both the study and control populations , Chlamydia antigen was more prevalent among younger women and non-contraceptive users .
	manualset3
95245	1	400057	5	NULL	NULL	0	NULL	cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In both cases , a clinical and laboratory pattern suggesting CSS was found before the HCV infection was discovered .
	manualset3
95246	2	400057	5	NULL	NULL	NULL	NULL	clinical and laboratory pattern	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In both cases , a clinical and laboratory pattern suggesting CSS was found before the HCV infection was discovered .
	manualset3
95247	3	400057	5	NULL	NULL	0	NULL	CSS 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In both cases , a clinical and laboratory pattern suggesting CSS was found before the HCV infection was discovered .
	manualset3
95248	4	400057	5	NULL	NULL	0	NULL	HCV infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In both cases , a clinical and laboratory pattern suggesting CSS was found before the HCV infection was discovered .
	manualset3
95249	1	400058	5	NULL	NULL	NULL	NULL	cases	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In both cases , the piperazine ring adopts an almost perfect chair conformation and the benzoxazolinone ring system lies nearly perpendicular to it .
	manualset3
95250	2	400058	5	NULL	NULL	0	NULL	piperazine ring	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In both cases , the piperazine ring adopts an almost perfect chair conformation and the benzoxazolinone ring system lies nearly perpendicular to it .
	manualset3
95251	3	400058	5	NULL	NULL	0	NULL	chair conformation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In both cases , the piperazine ring adopts an almost perfect chair conformation and the benzoxazolinone ring system lies nearly perpendicular to it .
	manualset3
95252	4	400058	5	NULL	NULL	0	NULL	benzoxazolinone ring system	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In both cases , the piperazine ring adopts an almost perfect chair conformation and the benzoxazolinone ring system lies nearly perpendicular to it .
	manualset3
95253	1	400059	5	NULL	NULL	NULL	NULL	cases 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In both cases immunohistochemical examination revealed positivity for cytokeratins CK7 and CK20 .
	manualset3
95254	2	400059	5	NULL	NULL	0	NULL	immunohistochemical examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In both cases immunohistochemical examination revealed positivity for cytokeratins CK7 and CK20 .
	manualset3
95255	3	400059	5	NULL	NULL	NULL	NULL	cytokeratins CK7 and CK20	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In both cases immunohistochemical examination revealed positivity for cytokeratins CK7 and CK20 .
	manualset3
95256	1	400060	5	NULL	NULL	0	NULL	groups of animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In both groups of animals , the cerebral blood flow of the ischemic cortex was significantly lower than that of the contralateral cortex ( 36 + / - 16 ( SD ) and 67 + / - 14 ml/min/100 g for the control group ; 33 + / - 10 and 58 + / - 11 ml/min/100 g for the MK-801 group , respectively ) .
	manualset3
95257	2	400060	5	NULL	NULL	0	NULL	cerebral blood flow	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In both groups of animals , the cerebral blood flow of the ischemic cortex was significantly lower than that of the contralateral cortex ( 36 + / - 16 ( SD ) and 67 + / - 14 ml/min/100 g for the control group ; 33 + / - 10 and 58 + / - 11 ml/min/100 g for the MK-801 group , respectively ) .
	manualset3
95259	3	400060	5	NULL	NULL	0	NULL	ischemic cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In both groups of animals , the cerebral blood flow of the ischemic cortex was significantly lower than that of the contralateral cortex ( 36 + / - 16 ( SD ) and 67 + / - 14 ml/min/100 g for the control group ; 33 + / - 10 and 58 + / - 11 ml/min/100 g for the MK-801 group , respectively ) .
	manualset3
95260	4	400060	5	NULL	NULL	0	NULL	contralateral cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In both groups of animals , the cerebral blood flow of the ischemic cortex was significantly lower than that of the contralateral cortex ( 36 + / - 16 ( SD ) and 67 + / - 14 ml/min/100 g for the control group ; 33 + / - 10 and 58 + / - 11 ml/min/100 g for the MK-801 group , respectively ) .
	manualset3
95261	5	400060	5	NULL	NULL	0	NULL	( 36 + / - 16 ( SD ) and 67 + / - 14 ml/min/100 g for the control group ; 33 + / - 10 and 58 + / - 11 ml/min/100 g for the MK-801 group , respectively )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In both groups of animals , the cerebral blood flow of the ischemic cortex was significantly lower than that of the contralateral cortex ( 36 + / - 16 ( SD ) and 67 + / - 14 ml/min/100 g for the control group ; 33 + / - 10 and 58 + / - 11 ml/min/100 g for the MK-801 group , respectively ) .
	manualset3
95263	1	400061	5	NULL	NULL	0	NULL	groups of hypertensive rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In both groups of hypertensive rats the pressor response to injection into the nucleus tractus solitarius of the GABA uptake blocking drug nipecotic acid was significantly greater compared with control rats ( P & lt ; .01 in each model ) .
	manualset3
95264	2	400061	5	NULL	NULL	0	NULL	pressor response to injection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In both groups of hypertensive rats the pressor response to injection into the nucleus tractus solitarius of the GABA uptake blocking drug nipecotic acid was significantly greater compared with control rats ( P & lt ; .01 in each model ) .
	manualset3
95265	3	400061	5	NULL	NULL	0	NULL	nucleus tractus solitarius	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In both groups of hypertensive rats the pressor response to injection into the nucleus tractus solitarius of the GABA uptake blocking drug nipecotic acid was significantly greater compared with control rats ( P & lt ; .01 in each model ) .
	manualset3
95266	4	400061	5	NULL	NULL	0	NULL	GABA uptake blocking drug nipecotic acid	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In both groups of hypertensive rats the pressor response to injection into the nucleus tractus solitarius of the GABA uptake blocking drug nipecotic acid was significantly greater compared with control rats ( P & lt ; .01 in each model ) .
	manualset3
95267	5	400061	5	NULL	NULL	0	NULL	control rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In both groups of hypertensive rats the pressor response to injection into the nucleus tractus solitarius of the GABA uptake blocking drug nipecotic acid was significantly greater compared with control rats ( P & lt ; .01 in each model ) .
	manualset3
95269	6	400061	5	NULL	NULL	0	NULL	( P & lt ; .01 in each model )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In both groups of hypertensive rats the pressor response to injection into the nucleus tractus solitarius of the GABA uptake blocking drug nipecotic acid was significantly greater compared with control rats ( P & lt ; .01 in each model ) .
	manualset3
95271	1	400062	5	NULL	NULL	0	NULL	Vesicostomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Vesicostomy : a temporary urinary diversion in childhood ) .
	manualset3
95272	2	400062	5	NULL	NULL	0	NULL	temporary urinary diversion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Vesicostomy : a temporary urinary diversion in childhood ) .
	manualset3
95273	3	400062	5	NULL	NULL	0	NULL	childhood	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	( Vesicostomy : a temporary urinary diversion in childhood ) .
	manualset3
95276	1	400063	5	NULL	NULL	0	NULL	groups 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In both groups the calves were divided into four age categories : 7 to 10 days ( 7.8 % ) , 11 to 14 days ( 29.3 % ) , 15 to 21 days ( 53.0 % ) , 22 days and older ( 9.9 % ) .
	manualset3
95278	2	400063	5	NULL	NULL	0	NULL	calves	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In both groups the calves were divided into four age categories : 7 to 10 days ( 7.8 % ) , 11 to 14 days ( 29.3 % ) , 15 to 21 days ( 53.0 % ) , 22 days and older ( 9.9 % ) .
	manualset3
95281	3	400063	5	NULL	NULL	0	NULL	four age categories	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In both groups the calves were divided into four age categories : 7 to 10 days ( 7.8 % ) , 11 to 14 days ( 29.3 % ) , 15 to 21 days ( 53.0 % ) , 22 days and older ( 9.9 % ) .
	manualset3
95283	4	400063	5	NULL	NULL	0	NULL	7 to 10 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In both groups the calves were divided into four age categories : 7 to 10 days ( 7.8 % ) , 11 to 14 days ( 29.3 % ) , 15 to 21 days ( 53.0 % ) , 22 days and older ( 9.9 % ) .
	manualset3
95284	5	400063	5	NULL	NULL	0	NULL	( 7.8 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In both groups the calves were divided into four age categories : 7 to 10 days ( 7.8 % ) , 11 to 14 days ( 29.3 % ) , 15 to 21 days ( 53.0 % ) , 22 days and older ( 9.9 % ) .
	manualset3
95285	6	400063	5	NULL	NULL	0	NULL	11 to 14 days 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In both groups the calves were divided into four age categories : 7 to 10 days ( 7.8 % ) , 11 to 14 days ( 29.3 % ) , 15 to 21 days ( 53.0 % ) , 22 days and older ( 9.9 % ) .
	manualset3
95286	7	400063	5	NULL	NULL	0	NULL	( 29.3 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In both groups the calves were divided into four age categories : 7 to 10 days ( 7.8 % ) , 11 to 14 days ( 29.3 % ) , 15 to 21 days ( 53.0 % ) , 22 days and older ( 9.9 % ) .
	manualset3
95287	8	400063	5	NULL	NULL	0	NULL	15 to 21 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In both groups the calves were divided into four age categories : 7 to 10 days ( 7.8 % ) , 11 to 14 days ( 29.3 % ) , 15 to 21 days ( 53.0 % ) , 22 days and older ( 9.9 % ) .
	manualset3
95288	9	400063	5	NULL	NULL	0	NULL	( 53.0 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In both groups the calves were divided into four age categories : 7 to 10 days ( 7.8 % ) , 11 to 14 days ( 29.3 % ) , 15 to 21 days ( 53.0 % ) , 22 days and older ( 9.9 % ) .
	manualset3
95289	10	400063	5	NULL	NULL	0	NULL	22 days and older	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In both groups the calves were divided into four age categories : 7 to 10 days ( 7.8 % ) , 11 to 14 days ( 29.3 % ) , 15 to 21 days ( 53.0 % ) , 22 days and older ( 9.9 % ) .
	manualset3
95290	11	400063	5	NULL	NULL	0	NULL	 ( 9.9 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In both groups the calves were divided into four age categories : 7 to 10 days ( 7.8 % ) , 11 to 14 days ( 29.3 % ) , 15 to 21 days ( 53.0 % ) , 22 days and older ( 9.9 % ) .
	manualset3
95291	1	400064	5	NULL	NULL	0	NULL	sexes	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In both sexes , fertility preservation often means immature gametes cryopreservation .
	manualset3
95292	2	400064	5	NULL	NULL	NULL	NULL	fertility preservation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In both sexes , fertility preservation often means immature gametes cryopreservation .
	manualset3
95293	3	400064	5	NULL	NULL	0	NULL	immature gametes cryopreservation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In both sexes , fertility preservation often means immature gametes cryopreservation .
	manualset3
95294	1	400065	5	NULL	NULL	0	NULL	sexes 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In both sexes BMR significantly correlated with weight , BMI , and resistance index .
	manualset3
95295	2	400065	5	NULL	NULL	0	NULL	BMR	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In both sexes BMR significantly correlated with weight , BMI , and resistance index .
	manualset3
95296	3	400065	5	NULL	NULL	0	NULL	weight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In both sexes BMR significantly correlated with weight , BMI , and resistance index .
	manualset3
95297	4	400065	5	NULL	NULL	0	NULL	BMI	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In both sexes BMR significantly correlated with weight , BMI , and resistance index .
	manualset3
95298	5	400065	5	NULL	NULL	0	NULL	resistance index	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In both sexes BMR significantly correlated with weight , BMI , and resistance index .
	manualset3
95299	1	400066	5	NULL	NULL	0	NULL	 breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In breast cancer , maspin , a serine protease inhibitor , can suppress tumor growth and metastasis in vivo and tumor cell motility and invasion in vitro .
	manualset3
95300	2	400066	5	NULL	NULL	NULL	NULL	serine protease inhibitor	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In breast cancer , maspin , a serine protease inhibitor , can suppress tumor growth and metastasis in vivo and tumor cell motility and invasion in vitro .
	manualset3
95301	3	400066	5	NULL	NULL	NULL	NULL	tumor growth	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In breast cancer , maspin , a serine protease inhibitor , can suppress tumor growth and metastasis in vivo and tumor cell motility and invasion in vitro .
	manualset3
95302	4	400066	5	NULL	NULL	0	NULL	metastasis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In breast cancer , maspin , a serine protease inhibitor , can suppress tumor growth and metastasis in vivo and tumor cell motility and invasion in vitro .
	manualset3
95303	5	400066	5	NULL	NULL	0	NULL	tumor cell motility	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In breast cancer , maspin , a serine protease inhibitor , can suppress tumor growth and metastasis in vivo and tumor cell motility and invasion in vitro .
	manualset3
95304	6	400066	5	NULL	NULL	0	NULL	invasion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In breast cancer , maspin , a serine protease inhibitor , can suppress tumor growth and metastasis in vivo and tumor cell motility and invasion in vitro .
	manualset3
98568	7	400066	5	NULL	NULL	0	NULL	maspin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In breast cancer , maspin , a serine protease inhibitor , can suppress tumor growth and metastasis in vivo and tumor cell motility and invasion in vitro .
	manualset3
95305	1	400067	5	NULL	NULL	0	NULL	cancer immunotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In cancer immunotherapy , epitopes and variants derived from the MART-1 / Melan-A protein are widely used as clinical vaccines .
	manualset3
95306	2	400067	5	NULL	NULL	0	NULL	epitopes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In cancer immunotherapy , epitopes and variants derived from the MART-1 / Melan-A protein are widely used as clinical vaccines .
	manualset3
95307	3	400067	5	NULL	NULL	NULL	NULL	variants	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In cancer immunotherapy , epitopes and variants derived from the MART-1 / Melan-A protein are widely used as clinical vaccines .
	manualset3
95308	4	400067	5	NULL	NULL	0	NULL	MART-1 / Melan-A protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In cancer immunotherapy , epitopes and variants derived from the MART-1 / Melan-A protein are widely used as clinical vaccines .
	manualset3
95309	5	400067	5	NULL	NULL	0	NULL	clinical vaccines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In cancer immunotherapy , epitopes and variants derived from the MART-1 / Melan-A protein are widely used as clinical vaccines .
	manualset3
95310	1	400068	5	NULL	NULL	0	NULL	cardiac surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In cardiac surgery , contrast TEE has been reported to be useful in evaluating the adequacy of the delivery of cardioplegia as well as aiding in the detection of air emboli .
	manualset3
95345	2	400068	5	NULL	NULL	0	NULL	contrast TEE	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In cardiac surgery , contrast TEE has been reported to be useful in evaluating the adequacy of the delivery of cardioplegia as well as aiding in the detection of air emboli .
	manualset3
95349	3	400068	5	NULL	NULL	NULL	NULL	 delivery of cardioplegia	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In cardiac surgery , contrast TEE has been reported to be useful in evaluating the adequacy of the delivery of cardioplegia as well as aiding in the detection of air emboli .
	manualset3
95350	4	400068	5	NULL	NULL	0	NULL	detection of air emboli	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In cardiac surgery , contrast TEE has been reported to be useful in evaluating the adequacy of the delivery of cardioplegia as well as aiding in the detection of air emboli .
	manualset3
95351	1	400069	5	NULL	NULL	0	NULL	cardio-surgical patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In cardio-surgical patients , -- mainly functional class III -- we were unable to demonstrate any gross cardiovascular effects of large doses of methylprednisolone .
	manualset3
95355	2	400069	5	NULL	NULL	0	NULL	functional class III	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In cardio-surgical patients , -- mainly functional class III -- we were unable to demonstrate any gross cardiovascular effects of large doses of methylprednisolone .
	manualset3
95357	3	400069	5	NULL	NULL	0	NULL	gross cardiovascular effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In cardio-surgical patients , -- mainly functional class III -- we were unable to demonstrate any gross cardiovascular effects of large doses of methylprednisolone .
	manualset3
95358	4	400069	5	NULL	NULL	0	NULL	large doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In cardio-surgical patients , -- mainly functional class III -- we were unable to demonstrate any gross cardiovascular effects of large doses of methylprednisolone .
	manualset3
95360	5	400069	5	NULL	NULL	0	NULL	methylprednisolone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In cardio-surgical patients , -- mainly functional class III -- we were unable to demonstrate any gross cardiovascular effects of large doses of methylprednisolone .
	manualset3
95362	1	400070	5	NULL	NULL	0	NULL	gastric ulcer type I with superficial fundic gastritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In case of gastric ulcer type I with superficial fundic gastritis it emerges normozymogenism with hyperpepsinogenemia + + I , with preatrophic fundic gastritis hypozymogenism with normopepsinogenemia , with atrophic fundic gastritis hypozymogenism with hypopepsinogenemia I. In type II and III gastric ulcer the chief cell mass and serum pepsinogen I behavior as they do in duodenal ulcer with hyperpepsinogenemia although hypozymogenism is present .
	manualset3
95799	2	400070	5	NULL	NULL	0	NULL	normozymogenism with hyperpepsinogenemia + + I	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In case of gastric ulcer type I with superficial fundic gastritis it emerges normozymogenism with hyperpepsinogenemia + + I , with preatrophic fundic gastritis hypozymogenism with normopepsinogenemia , with atrophic fundic gastritis hypozymogenism with hypopepsinogenemia I. In type II and III gastric ulcer the chief cell mass and serum pepsinogen I behavior as they do in duodenal ulcer with hyperpepsinogenemia although hypozymogenism is present .
	manualset3
95800	3	400070	5	NULL	NULL	0	NULL	 preatrophic fundic gastritis hypozymogenism with normopepsinogenemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In case of gastric ulcer type I with superficial fundic gastritis it emerges normozymogenism with hyperpepsinogenemia + + I , with preatrophic fundic gastritis hypozymogenism with normopepsinogenemia , with atrophic fundic gastritis hypozymogenism with hypopepsinogenemia I. In type II and III gastric ulcer the chief cell mass and serum pepsinogen I behavior as they do in duodenal ulcer with hyperpepsinogenemia although hypozymogenism is present .
	manualset3
95801	4	400070	5	NULL	NULL	0	NULL	atrophic fundic gastritis hypozymogenism with hypopepsinogenemia I	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In case of gastric ulcer type I with superficial fundic gastritis it emerges normozymogenism with hyperpepsinogenemia + + I , with preatrophic fundic gastritis hypozymogenism with normopepsinogenemia , with atrophic fundic gastritis hypozymogenism with hypopepsinogenemia I. In type II and III gastric ulcer the chief cell mass and serum pepsinogen I behavior as they do in duodenal ulcer with hyperpepsinogenemia although hypozymogenism is present .
	manualset3
95802	5	400070	5	NULL	NULL	0	NULL	 type II gastric ulcer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In case of gastric ulcer type I with superficial fundic gastritis it emerges normozymogenism with hyperpepsinogenemia + + I , with preatrophic fundic gastritis hypozymogenism with normopepsinogenemia , with atrophic fundic gastritis hypozymogenism with hypopepsinogenemia I. In type II and III gastric ulcer the chief cell mass and serum pepsinogen I behavior as they do in duodenal ulcer with hyperpepsinogenemia although hypozymogenism is present .
	manualset3
95803	6	400070	5	NULL	NULL	0	NULL	type III gastric ulcer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In case of gastric ulcer type I with superficial fundic gastritis it emerges normozymogenism with hyperpepsinogenemia + + I , with preatrophic fundic gastritis hypozymogenism with normopepsinogenemia , with atrophic fundic gastritis hypozymogenism with hypopepsinogenemia I. In type II and III gastric ulcer the chief cell mass and serum pepsinogen I behavior as they do in duodenal ulcer with hyperpepsinogenemia although hypozymogenism is present .
	manualset3
95804	7	400070	5	NULL	NULL	0	NULL	cell mass	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In case of gastric ulcer type I with superficial fundic gastritis it emerges normozymogenism with hyperpepsinogenemia + + I , with preatrophic fundic gastritis hypozymogenism with normopepsinogenemia , with atrophic fundic gastritis hypozymogenism with hypopepsinogenemia I. In type II and III gastric ulcer the chief cell mass and serum pepsinogen I behavior as they do in duodenal ulcer with hyperpepsinogenemia although hypozymogenism is present .
	manualset3
95805	8	400070	5	NULL	NULL	0	NULL	serum pepsinogen I behavior	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In case of gastric ulcer type I with superficial fundic gastritis it emerges normozymogenism with hyperpepsinogenemia + + I , with preatrophic fundic gastritis hypozymogenism with normopepsinogenemia , with atrophic fundic gastritis hypozymogenism with hypopepsinogenemia I. In type II and III gastric ulcer the chief cell mass and serum pepsinogen I behavior as they do in duodenal ulcer with hyperpepsinogenemia although hypozymogenism is present .
	manualset3
95806	9	400070	5	NULL	NULL	0	NULL	duodenal ulcer with hyperpepsinogenemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In case of gastric ulcer type I with superficial fundic gastritis it emerges normozymogenism with hyperpepsinogenemia + + I , with preatrophic fundic gastritis hypozymogenism with normopepsinogenemia , with atrophic fundic gastritis hypozymogenism with hypopepsinogenemia I. In type II and III gastric ulcer the chief cell mass and serum pepsinogen I behavior as they do in duodenal ulcer with hyperpepsinogenemia although hypozymogenism is present .
	manualset3
95807	10	400070	5	NULL	NULL	0	NULL	hypozymogenism	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In case of gastric ulcer type I with superficial fundic gastritis it emerges normozymogenism with hyperpepsinogenemia + + I , with preatrophic fundic gastritis hypozymogenism with normopepsinogenemia , with atrophic fundic gastritis hypozymogenism with hypopepsinogenemia I. In type II and III gastric ulcer the chief cell mass and serum pepsinogen I behavior as they do in duodenal ulcer with hyperpepsinogenemia although hypozymogenism is present .
	manualset3
95808	1	400071	5	NULL	NULL	0	NULL	mission contraindications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In case that there are missing contraindications and an insufficient effect of the conventional medicamentous therapy the use of halothane in subnarcotic dosage with acute serious bronchial obstruction is indicated .
	manualset3
95809	2	400071	5	NULL	NULL	0	NULL	insufficient effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In case that there are missing contraindications and an insufficient effect of the conventional medicamentous therapy the use of halothane in subnarcotic dosage with acute serious bronchial obstruction is indicated .
	manualset3
95810	3	400071	5	NULL	NULL	0	NULL	conventional medicamentous therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In case that there are missing contraindications and an insufficient effect of the conventional medicamentous therapy the use of halothane in subnarcotic dosage with acute serious bronchial obstruction is indicated .
	manualset3
95811	4	400071	5	NULL	NULL	0	NULL	halothane 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In case that there are missing contraindications and an insufficient effect of the conventional medicamentous therapy the use of halothane in subnarcotic dosage with acute serious bronchial obstruction is indicated .
	manualset3
95812	5	400071	5	NULL	NULL	0	NULL	subnarcotic dosage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In case that there are missing contraindications and an insufficient effect of the conventional medicamentous therapy the use of halothane in subnarcotic dosage with acute serious bronchial obstruction is indicated .
	manualset3
95813	6	400071	5	NULL	NULL	0	NULL	acute serious bronchial obstruction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In case that there are missing contraindications and an insufficient effect of the conventional medicamentous therapy the use of halothane in subnarcotic dosage with acute serious bronchial obstruction is indicated .
	manualset3
95814	1	400072	5	NULL	NULL	0	NULL	mediastinal or intraabdominal visceral necrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In cases of mediastinal or intraabdominal visceral necrosis , steroid therapy , by depressing the patient 's ability to mount an inflammatory response , might worsen the injury and lead to life-threatening sepsis .
	manualset3
95815	2	400072	5	NULL	NULL	0	NULL	steroid therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In cases of mediastinal or intraabdominal visceral necrosis , steroid therapy , by depressing the patient 's ability to mount an inflammatory response , might worsen the injury and lead to life-threatening sepsis .
	manualset3
95816	3	400072	5	NULL	NULL	0	NULL	patient 's ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In cases of mediastinal or intraabdominal visceral necrosis , steroid therapy , by depressing the patient 's ability to mount an inflammatory response , might worsen the injury and lead to life-threatening sepsis .
	manualset3
95817	4	400072	5	NULL	NULL	0	NULL	inflammatory response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In cases of mediastinal or intraabdominal visceral necrosis , steroid therapy , by depressing the patient 's ability to mount an inflammatory response , might worsen the injury and lead to life-threatening sepsis .
	manualset3
95818	5	400072	5	NULL	NULL	0	NULL	injury 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In cases of mediastinal or intraabdominal visceral necrosis , steroid therapy , by depressing the patient 's ability to mount an inflammatory response , might worsen the injury and lead to life-threatening sepsis .
	manualset3
95819	6	400072	5	NULL	NULL	0	NULL	life-threatening sepsis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In cases of mediastinal or intraabdominal visceral necrosis , steroid therapy , by depressing the patient 's ability to mount an inflammatory response , might worsen the injury and lead to life-threatening sepsis .
	manualset3
95820	1	400073	5	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In cells of a lower eukaryote Saccharomyces cerevisiae , the expression of hybrid gene cry3aM-licBM2 ?
	manualset3
95821	2	400073	5	NULL	NULL	0	NULL	lower eukaryote Saccharomyces cerevisiae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In cells of a lower eukaryote Saccharomyces cerevisiae , the expression of hybrid gene cry3aM-licBM2 ?
	manualset3
95822	3	400073	5	NULL	NULL	0	NULL	expression 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In cells of a lower eukaryote Saccharomyces cerevisiae , the expression of hybrid gene cry3aM-licBM2 ?
	manualset3
95823	4	400073	5	NULL	NULL	0	NULL	hybrid gene cry3aM-licBM2	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In cells of a lower eukaryote Saccharomyces cerevisiae , the expression of hybrid gene cry3aM-licBM2 ?
	manualset3
95824	1	400074	5	NULL	NULL	NULL	NULL	subgroups of patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In certain subgroups of patients , such as those with Type 2 diabetes , the prevalence of NAFLD , defined by ultrasound , may be as high as 70 % .
	manualset3
95825	2	400074	5	NULL	NULL	0	NULL	Type 2 diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In certain subgroups of patients , such as those with Type 2 diabetes , the prevalence of NAFLD , defined by ultrasound , may be as high as 70 % .
	manualset3
95826	3	400074	5	NULL	NULL	0	NULL	NAFLD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In certain subgroups of patients , such as those with Type 2 diabetes , the prevalence of NAFLD , defined by ultrasound , may be as high as 70 % .
	manualset3
95827	4	400074	5	NULL	NULL	0	NULL	ultrasound 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In certain subgroups of patients , such as those with Type 2 diabetes , the prevalence of NAFLD , defined by ultrasound , may be as high as 70 % .
	manualset3
95828	5	400074	5	NULL	NULL	0	NULL	70 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In certain subgroups of patients , such as those with Type 2 diabetes , the prevalence of NAFLD , defined by ultrasound , may be as high as 70 % .
	manualset3
95829	1	400075	5	NULL	NULL	0	NULL	cholesterol-depleted membranes 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In cholesterol-depleted membranes , cholesterol levels could be restored to those found in untreated membranes by incubation of the membranes with an MbetaCD-cholesterol complex , which correlated with a reversal of the cholesterol depletion-mediated decrease in the level of high-affinity binding .
	manualset3
95830	2	400075	5	NULL	NULL	0	NULL	cholesterol levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In cholesterol-depleted membranes , cholesterol levels could be restored to those found in untreated membranes by incubation of the membranes with an MbetaCD-cholesterol complex , which correlated with a reversal of the cholesterol depletion-mediated decrease in the level of high-affinity binding .
	manualset3
95831	3	400075	5	NULL	NULL	0	NULL	untreated membranes 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In cholesterol-depleted membranes , cholesterol levels could be restored to those found in untreated membranes by incubation of the membranes with an MbetaCD-cholesterol complex , which correlated with a reversal of the cholesterol depletion-mediated decrease in the level of high-affinity binding .
	manualset3
95832	4	400075	5	NULL	NULL	0	NULL	incubation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In cholesterol-depleted membranes , cholesterol levels could be restored to those found in untreated membranes by incubation of the membranes with an MbetaCD-cholesterol complex , which correlated with a reversal of the cholesterol depletion-mediated decrease in the level of high-affinity binding .
	manualset3
95833	5	400075	5	NULL	NULL	0	NULL	membranes 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In cholesterol-depleted membranes , cholesterol levels could be restored to those found in untreated membranes by incubation of the membranes with an MbetaCD-cholesterol complex , which correlated with a reversal of the cholesterol depletion-mediated decrease in the level of high-affinity binding .
	manualset3
95834	6	400075	5	NULL	NULL	0	NULL	MbetaCD-cholesterol complex	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In cholesterol-depleted membranes , cholesterol levels could be restored to those found in untreated membranes by incubation of the membranes with an MbetaCD-cholesterol complex , which correlated with a reversal of the cholesterol depletion-mediated decrease in the level of high-affinity binding .
	manualset3
95835	7	400075	5	NULL	NULL	NULL	NULL	cholesterol depletion-mediated decrease in the level of high-affinity binding	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In cholesterol-depleted membranes , cholesterol levels could be restored to those found in untreated membranes by incubation of the membranes with an MbetaCD-cholesterol complex , which correlated with a reversal of the cholesterol depletion-mediated decrease in the level of high-affinity binding .
	manualset3
95836	1	400076	5	NULL	NULL	0	NULL	chronic renal failure rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In chronic renal failure rats , PTH mRNA levels were elevated both per RNA and per DNA of parathyroid cells , suggesting increased PTH mRNA levels per cell .
	manualset3
95837	2	400076	5	NULL	NULL	0	NULL	PTH mRNA levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In chronic renal failure rats , PTH mRNA levels were elevated both per RNA and per DNA of parathyroid cells , suggesting increased PTH mRNA levels per cell .
	manualset3
95838	3	400076	5	NULL	NULL	0	NULL	RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In chronic renal failure rats , PTH mRNA levels were elevated both per RNA and per DNA of parathyroid cells , suggesting increased PTH mRNA levels per cell .
	manualset3
95839	4	400076	5	NULL	NULL	0	NULL	DNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In chronic renal failure rats , PTH mRNA levels were elevated both per RNA and per DNA of parathyroid cells , suggesting increased PTH mRNA levels per cell .
	manualset3
95840	5	400076	5	NULL	NULL	0	NULL	parathyroid cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In chronic renal failure rats , PTH mRNA levels were elevated both per RNA and per DNA of parathyroid cells , suggesting increased PTH mRNA levels per cell .
	manualset3
95841	6	400076	5	NULL	NULL	0	NULL	PTH mRNA levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In chronic renal failure rats , PTH mRNA levels were elevated both per RNA and per DNA of parathyroid cells , suggesting increased PTH mRNA levels per cell .
	manualset3
95842	7	400076	5	NULL	NULL	0	NULL	cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In chronic renal failure rats , PTH mRNA levels were elevated both per RNA and per DNA of parathyroid cells , suggesting increased PTH mRNA levels per cell .
	manualset3
95843	1	400077	5	NULL	NULL	0	NULL	Vigilance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Vigilance and motor activity ) .
	manualset3
95844	2	400077	5	NULL	NULL	0	NULL	motor activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Vigilance and motor activity ) .
	manualset3
95845	1	400078	5	NULL	NULL	0	NULL	chronically hypoxic animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In chronically hypoxic animals , only approximately 14 % of the endothelial cells were labeled on day 1 in small lung arteries and approximately 8 % were still labeled on day 14 .
	manualset3
95846	2	400078	5	NULL	NULL	0	NULL	14 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In chronically hypoxic animals , only approximately 14 % of the endothelial cells were labeled on day 1 in small lung arteries and approximately 8 % were still labeled on day 14 .
	manualset3
95847	3	400078	5	NULL	NULL	0	NULL	endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In chronically hypoxic animals , only approximately 14 % of the endothelial cells were labeled on day 1 in small lung arteries and approximately 8 % were still labeled on day 14 .
	manualset3
95848	4	400078	5	NULL	NULL	0	NULL	day 1	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In chronically hypoxic animals , only approximately 14 % of the endothelial cells were labeled on day 1 in small lung arteries and approximately 8 % were still labeled on day 14 .
	manualset3
95849	5	400078	5	NULL	NULL	0	NULL	 small lung arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In chronically hypoxic animals , only approximately 14 % of the endothelial cells were labeled on day 1 in small lung arteries and approximately 8 % were still labeled on day 14 .
	manualset3
95850	6	400078	5	NULL	NULL	0	NULL	8 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In chronically hypoxic animals , only approximately 14 % of the endothelial cells were labeled on day 1 in small lung arteries and approximately 8 % were still labeled on day 14 .
	manualset3
95851	7	400078	5	NULL	NULL	0	NULL	day 14	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In chronically hypoxic animals , only approximately 14 % of the endothelial cells were labeled on day 1 in small lung arteries and approximately 8 % were still labeled on day 14 .
	manualset3
95852	1	400079	5	NULL	NULL	0	NULL	clinical practice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In clinical practice , there is no evidence that topical indomethacin significantly inhibits the inflammatory response to cryotherapy .
	manualset3
95853	2	400079	5	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In clinical practice , there is no evidence that topical indomethacin significantly inhibits the inflammatory response to cryotherapy .
	manualset3
95854	3	400079	5	NULL	NULL	0	NULL	topical indomethacin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In clinical practice , there is no evidence that topical indomethacin significantly inhibits the inflammatory response to cryotherapy .
	manualset3
95855	4	400079	5	NULL	NULL	0	NULL	inflammatory response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In clinical practice , there is no evidence that topical indomethacin significantly inhibits the inflammatory response to cryotherapy .
	manualset3
95856	5	400079	5	NULL	NULL	0	NULL	cryotherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In clinical practice , there is no evidence that topical indomethacin significantly inhibits the inflammatory response to cryotherapy .
	manualset3
95857	1	400080	5	NULL	NULL	NULL	NULL	alleles of C2	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In combination with alleles of C2 and BF they can be grouped into unique complotypes .
	manualset3
95858	2	400080	5	NULL	NULL	NULL	NULL	alleles of BF	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In combination with alleles of C2 and BF they can be grouped into unique complotypes .
	manualset3
95860	3	400080	5	NULL	NULL	NULL	NULL	unique complotypes	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In combination with alleles of C2 and BF they can be grouped into unique complotypes .
	manualset3
95861	1	400081	5	NULL	NULL	0	NULL	conventional X-ray examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In combination with conventional X-ray examination , sonography of the AC joint can be used at low cost and is easy to learn .
	manualset3
95862	2	400081	5	NULL	NULL	0	NULL	sonography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In combination with conventional X-ray examination , sonography of the AC joint can be used at low cost and is easy to learn .
	manualset3
95863	3	400081	5	NULL	NULL	0	NULL	 AC joint	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In combination with conventional X-ray examination , sonography of the AC joint can be used at low cost and is easy to learn .
	manualset3
95864	4	400081	5	NULL	NULL	0	NULL	low cost	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In combination with conventional X-ray examination , sonography of the AC joint can be used at low cost and is easy to learn .
	manualset3
95866	1	400082	5	NULL	NULL	0	NULL	combinations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In combinations differing at the IC subregion ( and other central regions , but not at the IA subregion ) between 60 and 100 % of first-set grafts were rejected , but some grafts survived for over 100 days .
	manualset3
95867	2	400082	5	NULL	NULL	NULL	NULL	IC subregion	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In combinations differing at the IC subregion ( and other central regions , but not at the IA subregion ) between 60 and 100 % of first-set grafts were rejected , but some grafts survived for over 100 days .
	manualset3
95868	3	400082	5	NULL	NULL	NULL	NULL	central regions	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In combinations differing at the IC subregion ( and other central regions , but not at the IA subregion ) between 60 and 100 % of first-set grafts were rejected , but some grafts survived for over 100 days .
	manualset3
95869	4	400082	5	NULL	NULL	0	NULL	IA subregion	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In combinations differing at the IC subregion ( and other central regions , but not at the IA subregion ) between 60 and 100 % of first-set grafts were rejected , but some grafts survived for over 100 days .
	manualset3
95870	5	400082	5	NULL	NULL	0	NULL	60 and 100 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In combinations differing at the IC subregion ( and other central regions , but not at the IA subregion ) between 60 and 100 % of first-set grafts were rejected , but some grafts survived for over 100 days .
	manualset3
95871	6	400082	5	NULL	NULL	NULL	NULL	first-set grafts	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In combinations differing at the IC subregion ( and other central regions , but not at the IA subregion ) between 60 and 100 % of first-set grafts were rejected , but some grafts survived for over 100 days .
	manualset3
95872	7	400082	5	NULL	NULL	0	NULL	grafts 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In combinations differing at the IC subregion ( and other central regions , but not at the IA subregion ) between 60 and 100 % of first-set grafts were rejected , but some grafts survived for over 100 days .
	manualset3
95873	8	400082	5	NULL	NULL	0	NULL	100 days	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In combinations differing at the IC subregion ( and other central regions , but not at the IA subregion ) between 60 and 100 % of first-set grafts were rejected , but some grafts survived for over 100 days .
	manualset3
95874	1	400083	5	NULL	NULL	0	NULL	combined hyperlipidemic ( type II B ) patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In combined hyperlipidemic ( type II B ) patients , triglyceride levels decreased by 45 percent , very low-density lipoprotein cholesterol levels decreased 52.7 percent , total cholesterol levels decreased 16 percent , low-density lipoprotein cholesterol levels decreased 6 percent , and high-density lipoprotein levels increased 15.3 percent for a low-density lipoprotein cholesterol : high-density lipoprotein cholesterol ratio decrease of 13 percent .
	manualset3
95875	2	400083	5	NULL	NULL	0	NULL	triglyceride levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In combined hyperlipidemic ( type II B ) patients , triglyceride levels decreased by 45 percent , very low-density lipoprotein cholesterol levels decreased 52.7 percent , total cholesterol levels decreased 16 percent , low-density lipoprotein cholesterol levels decreased 6 percent , and high-density lipoprotein levels increased 15.3 percent for a low-density lipoprotein cholesterol : high-density lipoprotein cholesterol ratio decrease of 13 percent .
	manualset3
95876	3	400083	5	NULL	NULL	0	NULL	45 percent	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In combined hyperlipidemic ( type II B ) patients , triglyceride levels decreased by 45 percent , very low-density lipoprotein cholesterol levels decreased 52.7 percent , total cholesterol levels decreased 16 percent , low-density lipoprotein cholesterol levels decreased 6 percent , and high-density lipoprotein levels increased 15.3 percent for a low-density lipoprotein cholesterol : high-density lipoprotein cholesterol ratio decrease of 13 percent .
	manualset3
95877	4	400083	5	NULL	NULL	0	NULL	very low-density lipoprotein cholesterol levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In combined hyperlipidemic ( type II B ) patients , triglyceride levels decreased by 45 percent , very low-density lipoprotein cholesterol levels decreased 52.7 percent , total cholesterol levels decreased 16 percent , low-density lipoprotein cholesterol levels decreased 6 percent , and high-density lipoprotein levels increased 15.3 percent for a low-density lipoprotein cholesterol : high-density lipoprotein cholesterol ratio decrease of 13 percent .
	manualset3
95878	5	400083	5	NULL	NULL	0	NULL	52.7 percent	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In combined hyperlipidemic ( type II B ) patients , triglyceride levels decreased by 45 percent , very low-density lipoprotein cholesterol levels decreased 52.7 percent , total cholesterol levels decreased 16 percent , low-density lipoprotein cholesterol levels decreased 6 percent , and high-density lipoprotein levels increased 15.3 percent for a low-density lipoprotein cholesterol : high-density lipoprotein cholesterol ratio decrease of 13 percent .
	manualset3
95879	6	400083	5	NULL	NULL	0	NULL	total cholesterol levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In combined hyperlipidemic ( type II B ) patients , triglyceride levels decreased by 45 percent , very low-density lipoprotein cholesterol levels decreased 52.7 percent , total cholesterol levels decreased 16 percent , low-density lipoprotein cholesterol levels decreased 6 percent , and high-density lipoprotein levels increased 15.3 percent for a low-density lipoprotein cholesterol : high-density lipoprotein cholesterol ratio decrease of 13 percent .
	manualset3
95880	7	400083	5	NULL	NULL	0	NULL	16 percent	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In combined hyperlipidemic ( type II B ) patients , triglyceride levels decreased by 45 percent , very low-density lipoprotein cholesterol levels decreased 52.7 percent , total cholesterol levels decreased 16 percent , low-density lipoprotein cholesterol levels decreased 6 percent , and high-density lipoprotein levels increased 15.3 percent for a low-density lipoprotein cholesterol : high-density lipoprotein cholesterol ratio decrease of 13 percent .
	manualset3
95881	8	400083	5	NULL	NULL	0	NULL	low-density lipoprotein cholesterol levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In combined hyperlipidemic ( type II B ) patients , triglyceride levels decreased by 45 percent , very low-density lipoprotein cholesterol levels decreased 52.7 percent , total cholesterol levels decreased 16 percent , low-density lipoprotein cholesterol levels decreased 6 percent , and high-density lipoprotein levels increased 15.3 percent for a low-density lipoprotein cholesterol : high-density lipoprotein cholesterol ratio decrease of 13 percent .
	manualset3
95882	9	400083	5	NULL	NULL	0	NULL	6 percent	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In combined hyperlipidemic ( type II B ) patients , triglyceride levels decreased by 45 percent , very low-density lipoprotein cholesterol levels decreased 52.7 percent , total cholesterol levels decreased 16 percent , low-density lipoprotein cholesterol levels decreased 6 percent , and high-density lipoprotein levels increased 15.3 percent for a low-density lipoprotein cholesterol : high-density lipoprotein cholesterol ratio decrease of 13 percent .
	manualset3
95883	10	400083	5	NULL	NULL	0	NULL	 high-density lipoprotein levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In combined hyperlipidemic ( type II B ) patients , triglyceride levels decreased by 45 percent , very low-density lipoprotein cholesterol levels decreased 52.7 percent , total cholesterol levels decreased 16 percent , low-density lipoprotein cholesterol levels decreased 6 percent , and high-density lipoprotein levels increased 15.3 percent for a low-density lipoprotein cholesterol : high-density lipoprotein cholesterol ratio decrease of 13 percent .
	manualset3
95884	11	400083	5	NULL	NULL	0	NULL	 15.3 percent	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In combined hyperlipidemic ( type II B ) patients , triglyceride levels decreased by 45 percent , very low-density lipoprotein cholesterol levels decreased 52.7 percent , total cholesterol levels decreased 16 percent , low-density lipoprotein cholesterol levels decreased 6 percent , and high-density lipoprotein levels increased 15.3 percent for a low-density lipoprotein cholesterol : high-density lipoprotein cholesterol ratio decrease of 13 percent .
	manualset3
95885	12	400083	5	NULL	NULL	0	NULL	low-density lipoprotein cholesterol : high-density lipoprotein cholesterol ratio 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In combined hyperlipidemic ( type II B ) patients , triglyceride levels decreased by 45 percent , very low-density lipoprotein cholesterol levels decreased 52.7 percent , total cholesterol levels decreased 16 percent , low-density lipoprotein cholesterol levels decreased 6 percent , and high-density lipoprotein levels increased 15.3 percent for a low-density lipoprotein cholesterol : high-density lipoprotein cholesterol ratio decrease of 13 percent .
	manualset3
95886	13	400083	5	NULL	NULL	0	NULL	13 percent	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In combined hyperlipidemic ( type II B ) patients , triglyceride levels decreased by 45 percent , very low-density lipoprotein cholesterol levels decreased 52.7 percent , total cholesterol levels decreased 16 percent , low-density lipoprotein cholesterol levels decreased 6 percent , and high-density lipoprotein levels increased 15.3 percent for a low-density lipoprotein cholesterol : high-density lipoprotein cholesterol ratio decrease of 13 percent .
	manualset3
95887	1	400084	5	NULL	NULL	0	NULL	comparison	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with TFA , the HFB leaving group is a better nucleofuge for less than 0.5 unit of N ( f ) .
	manualset3
95888	2	400084	5	NULL	NULL	0	NULL	TFA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with TFA , the HFB leaving group is a better nucleofuge for less than 0.5 unit of N ( f ) .
	manualset3
95889	3	400084	5	NULL	NULL	0	NULL	HFB leaving group	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with TFA , the HFB leaving group is a better nucleofuge for less than 0.5 unit of N ( f ) .
	manualset3
95890	4	400084	5	NULL	NULL	0	NULL	nucleofuge 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with TFA , the HFB leaving group is a better nucleofuge for less than 0.5 unit of N ( f ) .
	manualset3
95891	5	400084	5	NULL	NULL	0	NULL	0.5 unit of N ( f )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with TFA , the HFB leaving group is a better nucleofuge for less than 0.5 unit of N ( f ) .
	manualset3
95892	1	400085	5	NULL	NULL	0	NULL	Visceral changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Visceral changes in scleroderma ) .
	manualset3
95894	2	400085	5	NULL	NULL	0	NULL	scleroderma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Visceral changes in scleroderma ) .
	manualset3
96339	1	400086	5	NULL	NULL	0	NULL	comparison	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with healthy elderly volunteers ( n = 25 ) , serum vitamin K1 concentrations were significantly lower in both groups at presentation , and fell significantly within 24 h after surgery to concentrations approaching non-detectable , subsequently returning to pre-operative values within 3 weeks .
	manualset3
96340	2	400086	5	NULL	NULL	0	NULL	healthy elderly volunteers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with healthy elderly volunteers ( n = 25 ) , serum vitamin K1 concentrations were significantly lower in both groups at presentation , and fell significantly within 24 h after surgery to concentrations approaching non-detectable , subsequently returning to pre-operative values within 3 weeks .
	manualset3
96341	3	400086	5	NULL	NULL	0	NULL	( n = 25 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with healthy elderly volunteers ( n = 25 ) , serum vitamin K1 concentrations were significantly lower in both groups at presentation , and fell significantly within 24 h after surgery to concentrations approaching non-detectable , subsequently returning to pre-operative values within 3 weeks .
	manualset3
96342	4	400086	5	NULL	NULL	0	NULL	serum vitamin K1 concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with healthy elderly volunteers ( n = 25 ) , serum vitamin K1 concentrations were significantly lower in both groups at presentation , and fell significantly within 24 h after surgery to concentrations approaching non-detectable , subsequently returning to pre-operative values within 3 weeks .
	manualset3
96343	5	400086	5	NULL	NULL	0	NULL	groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with healthy elderly volunteers ( n = 25 ) , serum vitamin K1 concentrations were significantly lower in both groups at presentation , and fell significantly within 24 h after surgery to concentrations approaching non-detectable , subsequently returning to pre-operative values within 3 weeks .
	manualset3
96344	6	400086	5	NULL	NULL	0	NULL	presentation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with healthy elderly volunteers ( n = 25 ) , serum vitamin K1 concentrations were significantly lower in both groups at presentation , and fell significantly within 24 h after surgery to concentrations approaching non-detectable , subsequently returning to pre-operative values within 3 weeks .
	manualset3
96345	7	400086	5	NULL	NULL	0	NULL	24 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with healthy elderly volunteers ( n = 25 ) , serum vitamin K1 concentrations were significantly lower in both groups at presentation , and fell significantly within 24 h after surgery to concentrations approaching non-detectable , subsequently returning to pre-operative values within 3 weeks .
	manualset3
96346	8	400086	5	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with healthy elderly volunteers ( n = 25 ) , serum vitamin K1 concentrations were significantly lower in both groups at presentation , and fell significantly within 24 h after surgery to concentrations approaching non-detectable , subsequently returning to pre-operative values within 3 weeks .
	manualset3
96347	9	400086	5	NULL	NULL	0	NULL	concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with healthy elderly volunteers ( n = 25 ) , serum vitamin K1 concentrations were significantly lower in both groups at presentation , and fell significantly within 24 h after surgery to concentrations approaching non-detectable , subsequently returning to pre-operative values within 3 weeks .
	manualset3
96348	10	400086	5	NULL	NULL	0	NULL	pre-operative values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with healthy elderly volunteers ( n = 25 ) , serum vitamin K1 concentrations were significantly lower in both groups at presentation , and fell significantly within 24 h after surgery to concentrations approaching non-detectable , subsequently returning to pre-operative values within 3 weeks .
	manualset3
96349	11	400086	5	NULL	NULL	0	NULL	3 weeks	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with healthy elderly volunteers ( n = 25 ) , serum vitamin K1 concentrations were significantly lower in both groups at presentation , and fell significantly within 24 h after surgery to concentrations approaching non-detectable , subsequently returning to pre-operative values within 3 weeks .
	manualset3
96350	1	400087	5	NULL	NULL	0	NULL	comparison 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with plasma , only few amino acids have higher levels in red cells : aspartic and glutamic acids , glycine .
	manualset3
96351	2	400087	5	NULL	NULL	0	NULL	plasma	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with plasma , only few amino acids have higher levels in red cells : aspartic and glutamic acids , glycine .
	manualset3
96352	3	400087	5	NULL	NULL	0	NULL	amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with plasma , only few amino acids have higher levels in red cells : aspartic and glutamic acids , glycine .
	manualset3
96353	4	400087	5	NULL	NULL	0	NULL	higher levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with plasma , only few amino acids have higher levels in red cells : aspartic and glutamic acids , glycine .
	manualset3
96354	5	400087	5	NULL	NULL	0	NULL	red cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with plasma , only few amino acids have higher levels in red cells : aspartic and glutamic acids , glycine .
	manualset3
96355	6	400087	5	NULL	NULL	0	NULL	aspartic acid	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with plasma , only few amino acids have higher levels in red cells : aspartic and glutamic acids , glycine .
	manualset3
96356	7	400087	5	NULL	NULL	0	NULL	glutamic acid	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with plasma , only few amino acids have higher levels in red cells : aspartic and glutamic acids , glycine .
	manualset3
96357	8	400087	5	NULL	NULL	0	NULL	glycine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with plasma , only few amino acids have higher levels in red cells : aspartic and glutamic acids , glycine .
	manualset3
96358	1	400088	5	NULL	NULL	0	NULL	competition experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In competition experiments murine p53 replaced human p53 ( hp53 ) in p53-DNA complexes and this correlated with the greater lability observed for hp53-DNA complexes at a given temperature .
	manualset3
96359	2	400088	5	NULL	NULL	0	NULL	murine p53	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In competition experiments murine p53 replaced human p53 ( hp53 ) in p53-DNA complexes and this correlated with the greater lability observed for hp53-DNA complexes at a given temperature .
	manualset3
96360	3	400088	5	NULL	NULL	0	NULL	human p53 ( hp53 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In competition experiments murine p53 replaced human p53 ( hp53 ) in p53-DNA complexes and this correlated with the greater lability observed for hp53-DNA complexes at a given temperature .
	manualset3
96361	4	400088	5	NULL	NULL	NULL	NULL	p53-DNA complexes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In competition experiments murine p53 replaced human p53 ( hp53 ) in p53-DNA complexes and this correlated with the greater lability observed for hp53-DNA complexes at a given temperature .
	manualset3
96362	5	400088	5	NULL	NULL	0	NULL	lability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In competition experiments murine p53 replaced human p53 ( hp53 ) in p53-DNA complexes and this correlated with the greater lability observed for hp53-DNA complexes at a given temperature .
	manualset3
96363	6	400088	5	NULL	NULL	NULL	NULL	hp53-DNA complexes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In competition experiments murine p53 replaced human p53 ( hp53 ) in p53-DNA complexes and this correlated with the greater lability observed for hp53-DNA complexes at a given temperature .
	manualset3
96364	7	400088	5	NULL	NULL	0	NULL	temperature 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In competition experiments murine p53 replaced human p53 ( hp53 ) in p53-DNA complexes and this correlated with the greater lability observed for hp53-DNA complexes at a given temperature .
	manualset3
96365	1	400089	5	NULL	NULL	0	NULL	concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In concentrations in the range found in man during valproate therapy ( 0.1-1 .0 mM ) , it inhibited pyruvate and palmitate oxidation , urea synthesis and gluconeogenesis by 30-50 % in isolated rat hepatocytes .
	manualset3
96366	2	400089	5	NULL	NULL	0	NULL	range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In concentrations in the range found in man during valproate therapy ( 0.1-1 .0 mM ) , it inhibited pyruvate and palmitate oxidation , urea synthesis and gluconeogenesis by 30-50 % in isolated rat hepatocytes .
	manualset3
96367	3	400089	5	NULL	NULL	0	NULL	man	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In concentrations in the range found in man during valproate therapy ( 0.1-1 .0 mM ) , it inhibited pyruvate and palmitate oxidation , urea synthesis and gluconeogenesis by 30-50 % in isolated rat hepatocytes .
	manualset3
96368	4	400089	5	NULL	NULL	0	NULL	valproate therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In concentrations in the range found in man during valproate therapy ( 0.1-1 .0 mM ) , it inhibited pyruvate and palmitate oxidation , urea synthesis and gluconeogenesis by 30-50 % in isolated rat hepatocytes .
	manualset3
96369	5	400089	5	NULL	NULL	0	NULL	( 0.1-1 .0 mM )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In concentrations in the range found in man during valproate therapy ( 0.1-1 .0 mM ) , it inhibited pyruvate and palmitate oxidation , urea synthesis and gluconeogenesis by 30-50 % in isolated rat hepatocytes .
	manualset3
96370	6	400089	5	NULL	NULL	0	NULL	pyruvate oxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In concentrations in the range found in man during valproate therapy ( 0.1-1 .0 mM ) , it inhibited pyruvate and palmitate oxidation , urea synthesis and gluconeogenesis by 30-50 % in isolated rat hepatocytes .
	manualset3
96371	7	400089	5	NULL	NULL	0	NULL	palmitate oxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In concentrations in the range found in man during valproate therapy ( 0.1-1 .0 mM ) , it inhibited pyruvate and palmitate oxidation , urea synthesis and gluconeogenesis by 30-50 % in isolated rat hepatocytes .
	manualset3
96372	8	400089	5	NULL	NULL	0	NULL	urea synthesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In concentrations in the range found in man during valproate therapy ( 0.1-1 .0 mM ) , it inhibited pyruvate and palmitate oxidation , urea synthesis and gluconeogenesis by 30-50 % in isolated rat hepatocytes .
	manualset3
96373	9	400089	5	NULL	NULL	0	NULL	gluconeogenesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In concentrations in the range found in man during valproate therapy ( 0.1-1 .0 mM ) , it inhibited pyruvate and palmitate oxidation , urea synthesis and gluconeogenesis by 30-50 % in isolated rat hepatocytes .
	manualset3
96374	10	400089	5	NULL	NULL	0	NULL	30-50 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In concentrations in the range found in man during valproate therapy ( 0.1-1 .0 mM ) , it inhibited pyruvate and palmitate oxidation , urea synthesis and gluconeogenesis by 30-50 % in isolated rat hepatocytes .
	manualset3
96375	11	400089	5	NULL	NULL	0	NULL	isolated rat hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In concentrations in the range found in man during valproate therapy ( 0.1-1 .0 mM ) , it inhibited pyruvate and palmitate oxidation , urea synthesis and gluconeogenesis by 30-50 % in isolated rat hepatocytes .
	manualset3
96376	1	400090	5	NULL	NULL	0	NULL	conclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion : ( i ) FK228 showed a suppressive effect on the expression of angiogenesis factors , such as VEGF and bFGF , in PC-3 xenograft but not in ACHN xenograft , which suggests that the effect on the expression of angiogenesis factors is important for the antitumor efficacy of FK228 ; ( ii ) FK228 caused histone acetylation of the VEGF promoter regions , which may contribute to the suppression of VEGF gene expression .
	manualset3
96377	2	400090	5	NULL	NULL	0	NULL	FK228	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion : ( i ) FK228 showed a suppressive effect on the expression of angiogenesis factors , such as VEGF and bFGF , in PC-3 xenograft but not in ACHN xenograft , which suggests that the effect on the expression of angiogenesis factors is important for the antitumor efficacy of FK228 ; ( ii ) FK228 caused histone acetylation of the VEGF promoter regions , which may contribute to the suppression of VEGF gene expression .
	manualset3
96378	3	400090	5	NULL	NULL	0	NULL	 suppressive effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion : ( i ) FK228 showed a suppressive effect on the expression of angiogenesis factors , such as VEGF and bFGF , in PC-3 xenograft but not in ACHN xenograft , which suggests that the effect on the expression of angiogenesis factors is important for the antitumor efficacy of FK228 ; ( ii ) FK228 caused histone acetylation of the VEGF promoter regions , which may contribute to the suppression of VEGF gene expression .
	manualset3
96379	4	400090	5	NULL	NULL	NULL	NULL	expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion : ( i ) FK228 showed a suppressive effect on the expression of angiogenesis factors , such as VEGF and bFGF , in PC-3 xenograft but not in ACHN xenograft , which suggests that the effect on the expression of angiogenesis factors is important for the antitumor efficacy of FK228 ; ( ii ) FK228 caused histone acetylation of the VEGF promoter regions , which may contribute to the suppression of VEGF gene expression .
	manualset3
96380	5	400090	5	NULL	NULL	0	NULL	angiogenesis factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion : ( i ) FK228 showed a suppressive effect on the expression of angiogenesis factors , such as VEGF and bFGF , in PC-3 xenograft but not in ACHN xenograft , which suggests that the effect on the expression of angiogenesis factors is important for the antitumor efficacy of FK228 ; ( ii ) FK228 caused histone acetylation of the VEGF promoter regions , which may contribute to the suppression of VEGF gene expression .
	manualset3
96381	6	400090	5	NULL	NULL	0	NULL	VEGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion : ( i ) FK228 showed a suppressive effect on the expression of angiogenesis factors , such as VEGF and bFGF , in PC-3 xenograft but not in ACHN xenograft , which suggests that the effect on the expression of angiogenesis factors is important for the antitumor efficacy of FK228 ; ( ii ) FK228 caused histone acetylation of the VEGF promoter regions , which may contribute to the suppression of VEGF gene expression .
	manualset3
96382	7	400090	5	NULL	NULL	0	NULL	bFGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion : ( i ) FK228 showed a suppressive effect on the expression of angiogenesis factors , such as VEGF and bFGF , in PC-3 xenograft but not in ACHN xenograft , which suggests that the effect on the expression of angiogenesis factors is important for the antitumor efficacy of FK228 ; ( ii ) FK228 caused histone acetylation of the VEGF promoter regions , which may contribute to the suppression of VEGF gene expression .
	manualset3
96383	8	400090	5	NULL	NULL	0	NULL	PC-3 xenograft	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion : ( i ) FK228 showed a suppressive effect on the expression of angiogenesis factors , such as VEGF and bFGF , in PC-3 xenograft but not in ACHN xenograft , which suggests that the effect on the expression of angiogenesis factors is important for the antitumor efficacy of FK228 ; ( ii ) FK228 caused histone acetylation of the VEGF promoter regions , which may contribute to the suppression of VEGF gene expression .
	manualset3
96384	9	400090	5	NULL	NULL	0	NULL	ACHN xenograft 	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion : ( i ) FK228 showed a suppressive effect on the expression of angiogenesis factors , such as VEGF and bFGF , in PC-3 xenograft but not in ACHN xenograft , which suggests that the effect on the expression of angiogenesis factors is important for the antitumor efficacy of FK228 ; ( ii ) FK228 caused histone acetylation of the VEGF promoter regions , which may contribute to the suppression of VEGF gene expression .
	manualset3
96385	10	400090	5	NULL	NULL	0	NULL	effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion : ( i ) FK228 showed a suppressive effect on the expression of angiogenesis factors , such as VEGF and bFGF , in PC-3 xenograft but not in ACHN xenograft , which suggests that the effect on the expression of angiogenesis factors is important for the antitumor efficacy of FK228 ; ( ii ) FK228 caused histone acetylation of the VEGF promoter regions , which may contribute to the suppression of VEGF gene expression .
	manualset3
96386	11	400090	5	NULL	NULL	NULL	NULL	expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion : ( i ) FK228 showed a suppressive effect on the expression of angiogenesis factors , such as VEGF and bFGF , in PC-3 xenograft but not in ACHN xenograft , which suggests that the effect on the expression of angiogenesis factors is important for the antitumor efficacy of FK228 ; ( ii ) FK228 caused histone acetylation of the VEGF promoter regions , which may contribute to the suppression of VEGF gene expression .
	manualset3
96387	12	400090	5	NULL	NULL	0	NULL	angiogenesis factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion : ( i ) FK228 showed a suppressive effect on the expression of angiogenesis factors , such as VEGF and bFGF , in PC-3 xenograft but not in ACHN xenograft , which suggests that the effect on the expression of angiogenesis factors is important for the antitumor efficacy of FK228 ; ( ii ) FK228 caused histone acetylation of the VEGF promoter regions , which may contribute to the suppression of VEGF gene expression .
	manualset3
96388	13	400090	5	NULL	NULL	0	NULL	antitumor efficacy 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion : ( i ) FK228 showed a suppressive effect on the expression of angiogenesis factors , such as VEGF and bFGF , in PC-3 xenograft but not in ACHN xenograft , which suggests that the effect on the expression of angiogenesis factors is important for the antitumor efficacy of FK228 ; ( ii ) FK228 caused histone acetylation of the VEGF promoter regions , which may contribute to the suppression of VEGF gene expression .
	manualset3
96389	14	400090	5	NULL	NULL	0	NULL	FK228	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion : ( i ) FK228 showed a suppressive effect on the expression of angiogenesis factors , such as VEGF and bFGF , in PC-3 xenograft but not in ACHN xenograft , which suggests that the effect on the expression of angiogenesis factors is important for the antitumor efficacy of FK228 ; ( ii ) FK228 caused histone acetylation of the VEGF promoter regions , which may contribute to the suppression of VEGF gene expression .
	manualset3
96390	15	400090	5	NULL	NULL	0	NULL	FK228	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion : ( i ) FK228 showed a suppressive effect on the expression of angiogenesis factors , such as VEGF and bFGF , in PC-3 xenograft but not in ACHN xenograft , which suggests that the effect on the expression of angiogenesis factors is important for the antitumor efficacy of FK228 ; ( ii ) FK228 caused histone acetylation of the VEGF promoter regions , which may contribute to the suppression of VEGF gene expression .
	manualset3
96391	16	400090	5	NULL	NULL	0	NULL	histone acetylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion : ( i ) FK228 showed a suppressive effect on the expression of angiogenesis factors , such as VEGF and bFGF , in PC-3 xenograft but not in ACHN xenograft , which suggests that the effect on the expression of angiogenesis factors is important for the antitumor efficacy of FK228 ; ( ii ) FK228 caused histone acetylation of the VEGF promoter regions , which may contribute to the suppression of VEGF gene expression .
	manualset3
96392	17	400090	5	NULL	NULL	0	NULL	VEGF promoter regions	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion : ( i ) FK228 showed a suppressive effect on the expression of angiogenesis factors , such as VEGF and bFGF , in PC-3 xenograft but not in ACHN xenograft , which suggests that the effect on the expression of angiogenesis factors is important for the antitumor efficacy of FK228 ; ( ii ) FK228 caused histone acetylation of the VEGF promoter regions , which may contribute to the suppression of VEGF gene expression .
	manualset3
96393	18	400090	5	NULL	NULL	0	NULL	suppression 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion : ( i ) FK228 showed a suppressive effect on the expression of angiogenesis factors , such as VEGF and bFGF , in PC-3 xenograft but not in ACHN xenograft , which suggests that the effect on the expression of angiogenesis factors is important for the antitumor efficacy of FK228 ; ( ii ) FK228 caused histone acetylation of the VEGF promoter regions , which may contribute to the suppression of VEGF gene expression .
	manualset3
96394	19	400090	5	NULL	NULL	0	NULL	VEGF gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion : ( i ) FK228 showed a suppressive effect on the expression of angiogenesis factors , such as VEGF and bFGF , in PC-3 xenograft but not in ACHN xenograft , which suggests that the effect on the expression of angiogenesis factors is important for the antitumor efficacy of FK228 ; ( ii ) FK228 caused histone acetylation of the VEGF promoter regions , which may contribute to the suppression of VEGF gene expression .
	manualset3
96395	1	400091	5	NULL	NULL	0	NULL	conclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion a combination of contrast enhanced and unenhanced 3D MP-RAGE sequences is the technique of choice for the examination of ENT tumors near the base of the skull .
	manualset3
96396	2	400091	5	NULL	NULL	NULL	NULL	combination of contrast enhanced and unenhanced 3D MP-RAGE sequences	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion a combination of contrast enhanced and unenhanced 3D MP-RAGE sequences is the technique of choice for the examination of ENT tumors near the base of the skull .
	manualset3
96397	3	400091	5	NULL	NULL	NULL	NULL	technique	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In conclusion a combination of contrast enhanced and unenhanced 3D MP-RAGE sequences is the technique of choice for the examination of ENT tumors near the base of the skull .
	manualset3
96398	4	400091	5	NULL	NULL	0	NULL	examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion a combination of contrast enhanced and unenhanced 3D MP-RAGE sequences is the technique of choice for the examination of ENT tumors near the base of the skull .
	manualset3
96399	5	400091	5	NULL	NULL	0	NULL	ENT tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion a combination of contrast enhanced and unenhanced 3D MP-RAGE sequences is the technique of choice for the examination of ENT tumors near the base of the skull .
	manualset3
96400	6	400091	5	NULL	NULL	0	NULL	 base of the skull	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion a combination of contrast enhanced and unenhanced 3D MP-RAGE sequences is the technique of choice for the examination of ENT tumors near the base of the skull .
	manualset3
96401	1	400092	5	NULL	NULL	0	NULL	conclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion some propositions are brought up for discussion .
	manualset3
96402	2	400092	5	NULL	NULL	0	NULL	propositions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion some propositions are brought up for discussion .
	manualset3
96403	3	400092	5	NULL	NULL	0	NULL	discussion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion some propositions are brought up for discussion .
	manualset3
96404	1	400093	5	NULL	NULL	0	NULL	conjunction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conjunction with Experiment 1 this suggests that conflicting auditory-visual motion information of an intact human walker leads to interference and thereby delaying the response .
	manualset3
96405	2	400093	5	NULL	NULL	0	NULL	Experiment 1	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conjunction with Experiment 1 this suggests that conflicting auditory-visual motion information of an intact human walker leads to interference and thereby delaying the response .
	manualset3
96406	3	400093	5	NULL	NULL	0	NULL	auditory-visual motion information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In conjunction with Experiment 1 this suggests that conflicting auditory-visual motion information of an intact human walker leads to interference and thereby delaying the response .
	manualset3
96407	4	400093	5	NULL	NULL	0	NULL	intact human walker	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In conjunction with Experiment 1 this suggests that conflicting auditory-visual motion information of an intact human walker leads to interference and thereby delaying the response .
	manualset3
96408	5	400093	5	NULL	NULL	0	NULL	interference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conjunction with Experiment 1 this suggests that conflicting auditory-visual motion information of an intact human walker leads to interference and thereby delaying the response .
	manualset3
96409	6	400093	5	NULL	NULL	0	NULL	response	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conjunction with Experiment 1 this suggests that conflicting auditory-visual motion information of an intact human walker leads to interference and thereby delaying the response .
	manualset3
96410	1	400094	5	NULL	NULL	0	NULL	conjunction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conjunction with the downregulation of adhesion proteins , NK3 .3 cells cultured in the presence of cortisol exhibit a reduced capacity to form conjugates with K562 target cells .
	manualset3
96411	2	400094	5	NULL	NULL	0	NULL	downregulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conjunction with the downregulation of adhesion proteins , NK3 .3 cells cultured in the presence of cortisol exhibit a reduced capacity to form conjugates with K562 target cells .
	manualset3
96412	3	400094	5	NULL	NULL	0	NULL	adhesion proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In conjunction with the downregulation of adhesion proteins , NK3 .3 cells cultured in the presence of cortisol exhibit a reduced capacity to form conjugates with K562 target cells .
	manualset3
96413	4	400094	5	NULL	NULL	0	NULL	NK3 .3 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In conjunction with the downregulation of adhesion proteins , NK3 .3 cells cultured in the presence of cortisol exhibit a reduced capacity to form conjugates with K562 target cells .
	manualset3
96414	5	400094	5	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conjunction with the downregulation of adhesion proteins , NK3 .3 cells cultured in the presence of cortisol exhibit a reduced capacity to form conjugates with K562 target cells .
	manualset3
96415	6	400094	5	NULL	NULL	0	NULL	cortisol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In conjunction with the downregulation of adhesion proteins , NK3 .3 cells cultured in the presence of cortisol exhibit a reduced capacity to form conjugates with K562 target cells .
	manualset3
96416	7	400094	5	NULL	NULL	0	NULL	reduced capacity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conjunction with the downregulation of adhesion proteins , NK3 .3 cells cultured in the presence of cortisol exhibit a reduced capacity to form conjugates with K562 target cells .
	manualset3
96417	8	400094	5	NULL	NULL	0	NULL	conjugates	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conjunction with the downregulation of adhesion proteins , NK3 .3 cells cultured in the presence of cortisol exhibit a reduced capacity to form conjugates with K562 target cells .
	manualset3
96418	9	400094	5	NULL	NULL	0	NULL	K562 target cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In conjunction with the downregulation of adhesion proteins , NK3 .3 cells cultured in the presence of cortisol exhibit a reduced capacity to form conjugates with K562 target cells .
	manualset3
96419	1	400095	5	NULL	NULL	NULL	NULL	non-parasitic cyst	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Voluminous solitary non-parasitic cyst of the liver treated with marsupialization and following fistulo-entero-anastomosis ) .
	manualset3
96420	3	400095	5	NULL	NULL	NULL	NULL	marsupialization	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Voluminous solitary non-parasitic cyst of the liver treated with marsupialization and following fistulo-entero-anastomosis ) .
	manualset3
96421	2	400095	5	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Voluminous solitary non-parasitic cyst of the liver treated with marsupialization and following fistulo-entero-anastomosis ) .
	manualset3
96422	4	400095	5	NULL	NULL	0	NULL	fistulo-entero-anastomosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Voluminous solitary non-parasitic cyst of the liver treated with marsupialization and following fistulo-entero-anastomosis ) .
	manualset3
96423	1	400096	5	NULL	NULL	0	NULL	constant-infusion studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In constant-infusion studies , the bias error percent is shown to equal approximately the plateau enrichment , generally & lt ; 10 % .
	manualset3
96424	2	400096	5	NULL	NULL	0	NULL	bias error percent	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In constant-infusion studies , the bias error percent is shown to equal approximately the plateau enrichment , generally & lt ; 10 % .
	manualset3
96425	3	400096	5	NULL	NULL	NULL	NULL	plateau enrichment	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In constant-infusion studies , the bias error percent is shown to equal approximately the plateau enrichment , generally & lt ; 10 % .
	manualset3
96426	4	400096	5	NULL	NULL	0	NULL	10%	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In constant-infusion studies , the bias error percent is shown to equal approximately the plateau enrichment , generally & lt ; 10 % .
	manualset3
96427	1	400097	5	NULL	NULL	0	NULL	constant darkness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In constant darkness ( day 2 ) , the circadian melatonin rhythm in both the pineal gland and circulation was the same as that in untreated controls .
	manualset3
96428	2	400097	5	NULL	NULL	0	NULL	 ( day 2 )	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In constant darkness ( day 2 ) , the circadian melatonin rhythm in both the pineal gland and circulation was the same as that in untreated controls .
	manualset3
96429	3	400097	5	NULL	NULL	0	NULL	circadian melatonin rhythm	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In constant darkness ( day 2 ) , the circadian melatonin rhythm in both the pineal gland and circulation was the same as that in untreated controls .
	manualset3
96430	4	400097	5	NULL	NULL	0	NULL	pineal gland	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In constant darkness ( day 2 ) , the circadian melatonin rhythm in both the pineal gland and circulation was the same as that in untreated controls .
	manualset3
96431	5	400097	5	NULL	NULL	0	NULL	circulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In constant darkness ( day 2 ) , the circadian melatonin rhythm in both the pineal gland and circulation was the same as that in untreated controls .
	manualset3
96432	6	400097	5	NULL	NULL	0	NULL	 untreated controls	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In constant darkness ( day 2 ) , the circadian melatonin rhythm in both the pineal gland and circulation was the same as that in untreated controls .
	manualset3
96433	1	400098	5	NULL	NULL	NULL	NULL	frequent observations	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In context with the frequent observations of excessive iron ( Fe ) storage in captive black rhinoceroses ( Diceros bicornis ) , it has been suggested that both an excessive dietary Fe content and a lack of dietary Fe-chelating substances , such as tannins , is the underlying cause .
	manualset3
96434	2	400098	5	NULL	NULL	0	NULL	excessive iron ( Fe ) storage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In context with the frequent observations of excessive iron ( Fe ) storage in captive black rhinoceroses ( Diceros bicornis ) , it has been suggested that both an excessive dietary Fe content and a lack of dietary Fe-chelating substances , such as tannins , is the underlying cause .
	manualset3
96435	3	400098	5	NULL	NULL	0	NULL	captive black rhinoceroses ( Diceros bicornis )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In context with the frequent observations of excessive iron ( Fe ) storage in captive black rhinoceroses ( Diceros bicornis ) , it has been suggested that both an excessive dietary Fe content and a lack of dietary Fe-chelating substances , such as tannins , is the underlying cause .
	manualset3
96436	4	400098	5	NULL	NULL	0	NULL	excessive dietary Fe content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In context with the frequent observations of excessive iron ( Fe ) storage in captive black rhinoceroses ( Diceros bicornis ) , it has been suggested that both an excessive dietary Fe content and a lack of dietary Fe-chelating substances , such as tannins , is the underlying cause .
	manualset3
96437	5	400098	5	NULL	NULL	0	NULL	dietary Fe-chelating substances	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In context with the frequent observations of excessive iron ( Fe ) storage in captive black rhinoceroses ( Diceros bicornis ) , it has been suggested that both an excessive dietary Fe content and a lack of dietary Fe-chelating substances , such as tannins , is the underlying cause .
	manualset3
96438	6	400098	5	NULL	NULL	0	NULL	tannins	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In context with the frequent observations of excessive iron ( Fe ) storage in captive black rhinoceroses ( Diceros bicornis ) , it has been suggested that both an excessive dietary Fe content and a lack of dietary Fe-chelating substances , such as tannins , is the underlying cause .
	manualset3
96439	1	400099	5	NULL	NULL	0	NULL	17-day fetal grafts 	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , 17-day fetal grafts ( N = 20 ) grew 6.8 + / - 3.4 times , * while 15-day fetal grafts ( N = 28 ) grew 17.5 + / - 6.1 * times .
	manualset3
96440	2	400099	5	NULL	NULL	0	NULL	( N = 20 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , 17-day fetal grafts ( N = 20 ) grew 6.8 + / - 3.4 times , * while 15-day fetal grafts ( N = 28 ) grew 17.5 + / - 6.1 * times .
	manualset3
96441	3	400099	5	NULL	NULL	0	NULL	6.8 + / - 3.4 times	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , 17-day fetal grafts ( N = 20 ) grew 6.8 + / - 3.4 times , * while 15-day fetal grafts ( N = 28 ) grew 17.5 + / - 6.1 * times .
	manualset3
96442	4	400099	5	NULL	NULL	0	NULL	15-day fetal grafts	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , 17-day fetal grafts ( N = 20 ) grew 6.8 + / - 3.4 times , * while 15-day fetal grafts ( N = 28 ) grew 17.5 + / - 6.1 * times .
	manualset3
96443	5	400099	5	NULL	NULL	0	NULL	( N = 28 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , 17-day fetal grafts ( N = 20 ) grew 6.8 + / - 3.4 times , * while 15-day fetal grafts ( N = 28 ) grew 17.5 + / - 6.1 * times .
	manualset3
96444	6	400099	5	NULL	NULL	0	NULL	17.5 + / - 6.1 * times	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , 17-day fetal grafts ( N = 20 ) grew 6.8 + / - 3.4 times , * while 15-day fetal grafts ( N = 28 ) grew 17.5 + / - 6.1 * times .
	manualset3
96445	1	400100	5	NULL	NULL	0	NULL	17 out of 111 skin samples	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , 17 out of 111 skin samples were positive : the mutation frequency in positive samples was around 10 ( 7 ) -10 ( -6 ) ( 10-100 copies of mutant in 10 ( 8 ) wild-type Mt DNA ) .
	manualset3
96446	2	400100	5	NULL	NULL	0	NULL	mutation frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , 17 out of 111 skin samples were positive : the mutation frequency in positive samples was around 10 ( 7 ) -10 ( -6 ) ( 10-100 copies of mutant in 10 ( 8 ) wild-type Mt DNA ) .
	manualset3
96447	3	400100	5	NULL	NULL	0	NULL	positive samples	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , 17 out of 111 skin samples were positive : the mutation frequency in positive samples was around 10 ( 7 ) -10 ( -6 ) ( 10-100 copies of mutant in 10 ( 8 ) wild-type Mt DNA ) .
	manualset3
96448	4	400100	5	NULL	NULL	0	NULL	10 ( 7 ) -10 ( -6 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , 17 out of 111 skin samples were positive : the mutation frequency in positive samples was around 10 ( 7 ) -10 ( -6 ) ( 10-100 copies of mutant in 10 ( 8 ) wild-type Mt DNA ) .
	manualset3
96449	5	400100	5	NULL	NULL	0	NULL	10-100 copies	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , 17 out of 111 skin samples were positive : the mutation frequency in positive samples was around 10 ( 7 ) -10 ( -6 ) ( 10-100 copies of mutant in 10 ( 8 ) wild-type Mt DNA ) .
	manualset3
96450	6	400100	5	NULL	NULL	0	NULL	mutant	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , 17 out of 111 skin samples were positive : the mutation frequency in positive samples was around 10 ( 7 ) -10 ( -6 ) ( 10-100 copies of mutant in 10 ( 8 ) wild-type Mt DNA ) .
	manualset3
96451	7	400100	5	NULL	NULL	0	NULL	10 ( 8 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , 17 out of 111 skin samples were positive : the mutation frequency in positive samples was around 10 ( 7 ) -10 ( -6 ) ( 10-100 copies of mutant in 10 ( 8 ) wild-type Mt DNA ) .
	manualset3
96452	8	400100	5	NULL	NULL	0	NULL	wild-type Mt DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , 17 out of 111 skin samples were positive : the mutation frequency in positive samples was around 10 ( 7 ) -10 ( -6 ) ( 10-100 copies of mutant in 10 ( 8 ) wild-type Mt DNA ) .
	manualset3
96453	1	400101	5	NULL	NULL	0	NULL	5 of the 7 isolates	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , 5 of the 7 isolates from the Fisher 's syndrome patients belonged to PEN 2 : LIO 4 .
	manualset3
96454	2	400101	5	NULL	NULL	0	NULL	Fisher 's syndrome patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , 5 of the 7 isolates from the Fisher 's syndrome patients belonged to PEN 2 : LIO 4 .
	manualset3
96455	3	400101	5	NULL	NULL	0	NULL	PEN 2 : LIO 4	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , 5 of the 7 isolates from the Fisher 's syndrome patients belonged to PEN 2 : LIO 4 .
	manualset3
96456	1	400102	5	NULL	NULL	0	NULL	B7-H4 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , B7-H4 expression did not differ significantly between the tumor tissues derived from the stomach and liver and the normal tissues .
	manualset3
96457	2	400102	5	NULL	NULL	0	NULL	tumor tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , B7-H4 expression did not differ significantly between the tumor tissues derived from the stomach and liver and the normal tissues .
	manualset3
96458	3	400102	5	NULL	NULL	0	NULL	stomach	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , B7-H4 expression did not differ significantly between the tumor tissues derived from the stomach and liver and the normal tissues .
	manualset3
96459	4	400102	5	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , B7-H4 expression did not differ significantly between the tumor tissues derived from the stomach and liver and the normal tissues .
	manualset3
96460	5	400102	5	NULL	NULL	0	NULL	normal tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , B7-H4 expression did not differ significantly between the tumor tissues derived from the stomach and liver and the normal tissues .
	manualset3
96461	1	400103	5	NULL	NULL	0	NULL	C1214 bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , C1214 bacteria cause a mannose-sensitive agglutination of guinea pig erythrocytes , show a mannose-sensitive attachment to buccal epithelial cells , and attach to urinary mucus .
	manualset3
96462	2	400103	5	NULL	NULL	0	NULL	mannose-sensitive agglutination	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , C1214 bacteria cause a mannose-sensitive agglutination of guinea pig erythrocytes , show a mannose-sensitive attachment to buccal epithelial cells , and attach to urinary mucus .
	manualset3
96463	3	400103	5	NULL	NULL	0	NULL	guinea pig erythrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , C1214 bacteria cause a mannose-sensitive agglutination of guinea pig erythrocytes , show a mannose-sensitive attachment to buccal epithelial cells , and attach to urinary mucus .
	manualset3
96464	4	400103	5	NULL	NULL	0	NULL	mannose-sensitive attachment	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , C1214 bacteria cause a mannose-sensitive agglutination of guinea pig erythrocytes , show a mannose-sensitive attachment to buccal epithelial cells , and attach to urinary mucus .
	manualset3
96465	5	400103	5	NULL	NULL	0	NULL	buccal epithelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , C1214 bacteria cause a mannose-sensitive agglutination of guinea pig erythrocytes , show a mannose-sensitive attachment to buccal epithelial cells , and attach to urinary mucus .
	manualset3
96466	6	400103	5	NULL	NULL	0	NULL	urinary mucus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , C1214 bacteria cause a mannose-sensitive agglutination of guinea pig erythrocytes , show a mannose-sensitive attachment to buccal epithelial cells , and attach to urinary mucus .
	manualset3
96467	1	400104	5	NULL	NULL	0	NULL	W. F. Theunissen	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( W. F. Theunissen 's 50th year as physician ) .
	manualset3
96468	2	400104	5	NULL	NULL	0	NULL	50th year	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	( W. F. Theunissen 's 50th year as physician ) .
	manualset3
96469	3	400104	5	NULL	NULL	0	NULL	physician	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( W. F. Theunissen 's 50th year as physician ) .
	manualset3
96470	1	400105	5	NULL	NULL	0	NULL	CaM	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , CaM only enhanced BAPTA-AM-evoked SOC activity in inside-out patches .
	manualset3
96471	2	400105	5	NULL	NULL	0	NULL	BAPTA-AM-evoked SOC activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , CaM only enhanced BAPTA-AM-evoked SOC activity in inside-out patches .
	manualset3
96472	3	400105	5	NULL	NULL	0	NULL	inside-out patches	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , CaM only enhanced BAPTA-AM-evoked SOC activity in inside-out patches .
	manualset3
96473	1	400106	5	NULL	NULL	0	NULL	HT29 MTX10 ( -5 )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , HT29 MTX10 ( -5 ) , a highly differentiated mucus-secreting variant of HT29 obtained by methotrexate selection , was much more resistant to LAK cells than parental HT29 cells .
	manualset3
96474	2	400106	5	NULL	NULL	0	NULL	highly differentiated mucus-secreting variant of HT29	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , HT29 MTX10 ( -5 ) , a highly differentiated mucus-secreting variant of HT29 obtained by methotrexate selection , was much more resistant to LAK cells than parental HT29 cells .
	manualset3
96475	3	400106	5	NULL	NULL	0	NULL	methotrexate selection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , HT29 MTX10 ( -5 ) , a highly differentiated mucus-secreting variant of HT29 obtained by methotrexate selection , was much more resistant to LAK cells than parental HT29 cells .
	manualset3
96476	4	400106	5	NULL	NULL	0	NULL	LAK cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , HT29 MTX10 ( -5 ) , a highly differentiated mucus-secreting variant of HT29 obtained by methotrexate selection , was much more resistant to LAK cells than parental HT29 cells .
	manualset3
96477	5	400106	5	NULL	NULL	0	NULL	parental HT29 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , HT29 MTX10 ( -5 ) , a highly differentiated mucus-secreting variant of HT29 obtained by methotrexate selection , was much more resistant to LAK cells than parental HT29 cells .
	manualset3
96478	1	400107	5	NULL	NULL	NULL	NULL	JM1 cells transfected with S70A	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , JM1 cells transfected with S70A , resulting in expression of Bcl-2 protein that can not be phosphorylated , were not efficiently rescued from apoptosis by VEGF .
	manualset3
96479	2	400107	5	NULL	NULL	NULL	NULL	expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , JM1 cells transfected with S70A , resulting in expression of Bcl-2 protein that can not be phosphorylated , were not efficiently rescued from apoptosis by VEGF .
	manualset3
96480	3	400107	5	NULL	NULL	0	NULL	Bcl-2 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , JM1 cells transfected with S70A , resulting in expression of Bcl-2 protein that can not be phosphorylated , were not efficiently rescued from apoptosis by VEGF .
	manualset3
96481	4	400107	5	NULL	NULL	0	NULL	apoptosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , JM1 cells transfected with S70A , resulting in expression of Bcl-2 protein that can not be phosphorylated , were not efficiently rescued from apoptosis by VEGF .
	manualset3
96482	5	400107	5	NULL	NULL	0	NULL	VEGF 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , JM1 cells transfected with S70A , resulting in expression of Bcl-2 protein that can not be phosphorylated , were not efficiently rescued from apoptosis by VEGF .
	manualset3
96483	1	400108	5	NULL	NULL	NULL	NULL	JNK inhibitor	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , JNK inhibitor enhanced the As2O3-induced p21 activation , also in a dose-dependent fashion .
	manualset3
96484	2	400108	5	NULL	NULL	0	NULL	As2O3-induced p21 activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , JNK inhibitor enhanced the As2O3-induced p21 activation , also in a dose-dependent fashion .
	manualset3
96485	1	400109	5	NULL	NULL	0	NULL	MAP	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , MAP only increased from 112 + / - 2 to 150 + / - 5 mmHg in the 4A + congenic strain .
	manualset3
96486	2	400109	5	NULL	NULL	0	NULL	112 + / - 2 to 150 + / - 5 mmHg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , MAP only increased from 112 + / - 2 to 150 + / - 5 mmHg in the 4A + congenic strain .
	manualset3
96487	3	400109	5	NULL	NULL	0	NULL	4A + congenic strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , MAP only increased from 112 + / - 2 to 150 + / - 5 mmHg in the 4A + congenic strain .
	manualset3
96488	1	400110	5	NULL	NULL	0	NULL	Mills et al. 's model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , Mills et al. 's model is less refined and requires fitting an input parameter to give the correct magnitude of velocity but it successfully accounts for the variation in the discharge with slope for regime A for a wide range of slopes ( Mills , Loggia , and Tixier , Europhys .
	manualset3
96489	2	400110	5	NULL	NULL	0	NULL	input parameter	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , Mills et al. 's model is less refined and requires fitting an input parameter to give the correct magnitude of velocity but it successfully accounts for the variation in the discharge with slope for regime A for a wide range of slopes ( Mills , Loggia , and Tixier , Europhys .
	manualset3
96490	3	400110	5	NULL	NULL	0	NULL	correct magnitude of velocity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , Mills et al. 's model is less refined and requires fitting an input parameter to give the correct magnitude of velocity but it successfully accounts for the variation in the discharge with slope for regime A for a wide range of slopes ( Mills , Loggia , and Tixier , Europhys .
	manualset3
96491	4	400110	5	NULL	NULL	0	NULL	variation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , Mills et al. 's model is less refined and requires fitting an input parameter to give the correct magnitude of velocity but it successfully accounts for the variation in the discharge with slope for regime A for a wide range of slopes ( Mills , Loggia , and Tixier , Europhys .
	manualset3
96492	5	400110	5	NULL	NULL	0	NULL	discharge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , Mills et al. 's model is less refined and requires fitting an input parameter to give the correct magnitude of velocity but it successfully accounts for the variation in the discharge with slope for regime A for a wide range of slopes ( Mills , Loggia , and Tixier , Europhys .
	manualset3
96493	6	400110	5	NULL	NULL	0	NULL	regime A	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , Mills et al. 's model is less refined and requires fitting an input parameter to give the correct magnitude of velocity but it successfully accounts for the variation in the discharge with slope for regime A for a wide range of slopes ( Mills , Loggia , and Tixier , Europhys .
	manualset3
96494	7	400110	5	NULL	NULL	0	NULL	wide range of slopes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , Mills et al. 's model is less refined and requires fitting an input parameter to give the correct magnitude of velocity but it successfully accounts for the variation in the discharge with slope for regime A for a wide range of slopes ( Mills , Loggia , and Tixier , Europhys .
	manualset3
96495	8	400110	5	NULL	NULL	0	NULL	Mills	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , Mills et al. 's model is less refined and requires fitting an input parameter to give the correct magnitude of velocity but it successfully accounts for the variation in the discharge with slope for regime A for a wide range of slopes ( Mills , Loggia , and Tixier , Europhys .
	manualset3
96496	9	400110	5	NULL	NULL	0	NULL	Loggia 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , Mills et al. 's model is less refined and requires fitting an input parameter to give the correct magnitude of velocity but it successfully accounts for the variation in the discharge with slope for regime A for a wide range of slopes ( Mills , Loggia , and Tixier , Europhys .
	manualset3
96497	10	400110	5	NULL	NULL	0	NULL	Tixier	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , Mills et al. 's model is less refined and requires fitting an input parameter to give the correct magnitude of velocity but it successfully accounts for the variation in the discharge with slope for regime A for a wide range of slopes ( Mills , Loggia , and Tixier , Europhys .
	manualset3
96498	11	400110	5	NULL	NULL	0	NULL	Europhys	Journal												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , Mills et al. 's model is less refined and requires fitting an input parameter to give the correct magnitude of velocity but it successfully accounts for the variation in the discharge with slope for regime A for a wide range of slopes ( Mills , Loggia , and Tixier , Europhys .
	manualset3
96499	1	400111	5	NULL	NULL	0	NULL	PBMC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , PBMC from healthy CMV-seropositive donors did not have either measurable CMV-specific cytolysis or secretion of IFN-gamma without in vitro stimulation .
	manualset3
96500	2	400111	5	NULL	NULL	0	NULL	healthy CMV-seropositive donors	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , PBMC from healthy CMV-seropositive donors did not have either measurable CMV-specific cytolysis or secretion of IFN-gamma without in vitro stimulation .
	manualset3
96501	3	400111	5	NULL	NULL	0	NULL	measurable CMV-specific cytolysis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , PBMC from healthy CMV-seropositive donors did not have either measurable CMV-specific cytolysis or secretion of IFN-gamma without in vitro stimulation .
	manualset3
96502	4	400111	5	NULL	NULL	0	NULL	secretion of IFN-gamma	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , PBMC from healthy CMV-seropositive donors did not have either measurable CMV-specific cytolysis or secretion of IFN-gamma without in vitro stimulation .
	manualset3
96503	5	400111	5	NULL	NULL	0	NULL	in vitro stimulation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , PBMC from healthy CMV-seropositive donors did not have either measurable CMV-specific cytolysis or secretion of IFN-gamma without in vitro stimulation .
	manualset3
96504	1	400112	5	NULL	NULL	0	NULL	SV5 F protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , SV5 F protein exhibited a considerable degree of fusion activity when coexpressed with either NDV or HPIV-3 HN or with influenza virus HA , although the kinetics of fusion were two - to threefold higher when the homologous SV5 F and HN proteins were coexpressed .
	manualset3
96505	2	400112	5	NULL	NULL	0	NULL	fusion activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , SV5 F protein exhibited a considerable degree of fusion activity when coexpressed with either NDV or HPIV-3 HN or with influenza virus HA , although the kinetics of fusion were two - to threefold higher when the homologous SV5 F and HN proteins were coexpressed .
	manualset3
96506	3	400112	5	NULL	NULL	0	NULL	NDV HN	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , SV5 F protein exhibited a considerable degree of fusion activity when coexpressed with either NDV or HPIV-3 HN or with influenza virus HA , although the kinetics of fusion were two - to threefold higher when the homologous SV5 F and HN proteins were coexpressed .
	manualset3
96507	4	400112	5	NULL	NULL	0	NULL	HPIV-3 HN	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , SV5 F protein exhibited a considerable degree of fusion activity when coexpressed with either NDV or HPIV-3 HN or with influenza virus HA , although the kinetics of fusion were two - to threefold higher when the homologous SV5 F and HN proteins were coexpressed .
	manualset3
96508	5	400112	5	NULL	NULL	0	NULL	influenza virus HA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , SV5 F protein exhibited a considerable degree of fusion activity when coexpressed with either NDV or HPIV-3 HN or with influenza virus HA , although the kinetics of fusion were two - to threefold higher when the homologous SV5 F and HN proteins were coexpressed .
	manualset3
96509	6	400112	5	NULL	NULL	0	NULL	kinetics of fusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , SV5 F protein exhibited a considerable degree of fusion activity when coexpressed with either NDV or HPIV-3 HN or with influenza virus HA , although the kinetics of fusion were two - to threefold higher when the homologous SV5 F and HN proteins were coexpressed .
	manualset3
96511	7	400112	5	NULL	NULL	0	NULL	homologous SV5 F protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , SV5 F protein exhibited a considerable degree of fusion activity when coexpressed with either NDV or HPIV-3 HN or with influenza virus HA , although the kinetics of fusion were two - to threefold higher when the homologous SV5 F and HN proteins were coexpressed .
	manualset3
96512	8	400112	5	NULL	NULL	0	NULL	HN proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , SV5 F protein exhibited a considerable degree of fusion activity when coexpressed with either NDV or HPIV-3 HN or with influenza virus HA , although the kinetics of fusion were two - to threefold higher when the homologous SV5 F and HN proteins were coexpressed .
	manualset3
96513	1	400113	5	NULL	NULL	0	NULL	WKYMVm	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , WKYMVm caused the release of complement receptor 3 from secretory vesicles in neutrophils .
	manualset3
96515	2	400113	5	NULL	NULL	0	NULL	release 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , WKYMVm caused the release of complement receptor 3 from secretory vesicles in neutrophils .
	manualset3
96516	3	400113	5	NULL	NULL	0	NULL	complement receptor 3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , WKYMVm caused the release of complement receptor 3 from secretory vesicles in neutrophils .
	manualset3
96517	4	400113	5	NULL	NULL	0	NULL	secretory vesicles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , WKYMVm caused the release of complement receptor 3 from secretory vesicles in neutrophils .
	manualset3
96518	5	400113	5	NULL	NULL	0	NULL	neutrophils	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , WKYMVm caused the release of complement receptor 3 from secretory vesicles in neutrophils .
	manualset3
96520	1	400114	5	NULL	NULL	NULL	NULL	low one minute Apgar	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , a low one minute Apgar ( & lt ; 4 ) remained a significant risk factor , with odds ratios of 2.7 ( 95 % confidence interval ( CI ) 1.5 to 5.2 ) for neonatal death and 3.8 ( 95 % CI 1.4 to 10.4 ) for cerebral palsy .
	manualset3
96521	2	400114	5	NULL	NULL	0	NULL	 ( & lt ; 4 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , a low one minute Apgar ( & lt ; 4 ) remained a significant risk factor , with odds ratios of 2.7 ( 95 % confidence interval ( CI ) 1.5 to 5.2 ) for neonatal death and 3.8 ( 95 % CI 1.4 to 10.4 ) for cerebral palsy .
	manualset3
96522	3	400114	5	NULL	NULL	0	NULL	significant risk factor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , a low one minute Apgar ( & lt ; 4 ) remained a significant risk factor , with odds ratios of 2.7 ( 95 % confidence interval ( CI ) 1.5 to 5.2 ) for neonatal death and 3.8 ( 95 % CI 1.4 to 10.4 ) for cerebral palsy .
	manualset3
96523	4	400114	5	NULL	NULL	0	NULL	odds ratios	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , a low one minute Apgar ( & lt ; 4 ) remained a significant risk factor , with odds ratios of 2.7 ( 95 % confidence interval ( CI ) 1.5 to 5.2 ) for neonatal death and 3.8 ( 95 % CI 1.4 to 10.4 ) for cerebral palsy .
	manualset3
96524	5	400114	5	NULL	NULL	0	NULL	2.7	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , a low one minute Apgar ( & lt ; 4 ) remained a significant risk factor , with odds ratios of 2.7 ( 95 % confidence interval ( CI ) 1.5 to 5.2 ) for neonatal death and 3.8 ( 95 % CI 1.4 to 10.4 ) for cerebral palsy .
	manualset3
96525	6	400114	5	NULL	NULL	0	NULL	( 95 % confidence interval ( CI ) 1.5 to 5.2 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , a low one minute Apgar ( & lt ; 4 ) remained a significant risk factor , with odds ratios of 2.7 ( 95 % confidence interval ( CI ) 1.5 to 5.2 ) for neonatal death and 3.8 ( 95 % CI 1.4 to 10.4 ) for cerebral palsy .
	manualset3
96526	7	400114	5	NULL	NULL	0	NULL	neonatal death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , a low one minute Apgar ( & lt ; 4 ) remained a significant risk factor , with odds ratios of 2.7 ( 95 % confidence interval ( CI ) 1.5 to 5.2 ) for neonatal death and 3.8 ( 95 % CI 1.4 to 10.4 ) for cerebral palsy .
	manualset3
96527	8	400114	5	NULL	NULL	0	NULL	3.8	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , a low one minute Apgar ( & lt ; 4 ) remained a significant risk factor , with odds ratios of 2.7 ( 95 % confidence interval ( CI ) 1.5 to 5.2 ) for neonatal death and 3.8 ( 95 % CI 1.4 to 10.4 ) for cerebral palsy .
	manualset3
96528	9	400114	5	NULL	NULL	0	NULL	( 95 % CI 1.4 to 10.4 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , a low one minute Apgar ( & lt ; 4 ) remained a significant risk factor , with odds ratios of 2.7 ( 95 % confidence interval ( CI ) 1.5 to 5.2 ) for neonatal death and 3.8 ( 95 % CI 1.4 to 10.4 ) for cerebral palsy .
	manualset3
96530	10	400114	5	NULL	NULL	0	NULL	cerebral palsy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , a low one minute Apgar ( & lt ; 4 ) remained a significant risk factor , with odds ratios of 2.7 ( 95 % confidence interval ( CI ) 1.5 to 5.2 ) for neonatal death and 3.8 ( 95 % CI 1.4 to 10.4 ) for cerebral palsy .
	manualset3
96531	1	400115	5	NULL	NULL	0	NULL	abundant IGF-II mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , abundant IGF-II mRNA was found exclusively in GC , whereas the IGF-IIr gene was expressed in both thecal cells and GC .
	manualset3
96533	2	400115	5	NULL	NULL	0	NULL	GC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , abundant IGF-II mRNA was found exclusively in GC , whereas the IGF-IIr gene was expressed in both thecal cells and GC .
	manualset3
96535	3	400115	5	NULL	NULL	0	NULL	IGF-IIr gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , abundant IGF-II mRNA was found exclusively in GC , whereas the IGF-IIr gene was expressed in both thecal cells and GC .
	manualset3
96536	4	400115	5	NULL	NULL	0	NULL	thecal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , abundant IGF-II mRNA was found exclusively in GC , whereas the IGF-IIr gene was expressed in both thecal cells and GC .
	manualset3
96537	5	400115	5	NULL	NULL	0	NULL	GC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , abundant IGF-II mRNA was found exclusively in GC , whereas the IGF-IIr gene was expressed in both thecal cells and GC .
	manualset3
96539	1	400116	5	NULL	NULL	0	NULL	activation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , activation of PKG inhibits the activity of small GTPase Rac1 and its association with the effector protein IQGAP1 .
	manualset3
96541	2	400116	5	NULL	NULL	0	NULL	PKG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , activation of PKG inhibits the activity of small GTPase Rac1 and its association with the effector protein IQGAP1 .
	manualset3
96542	3	400116	5	NULL	NULL	0	NULL	activity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , activation of PKG inhibits the activity of small GTPase Rac1 and its association with the effector protein IQGAP1 .
	manualset3
96543	4	400116	5	NULL	NULL	0	NULL	small GTPase Rac1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , activation of PKG inhibits the activity of small GTPase Rac1 and its association with the effector protein IQGAP1 .
	manualset3
96544	5	400116	5	NULL	NULL	0	NULL	association 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , activation of PKG inhibits the activity of small GTPase Rac1 and its association with the effector protein IQGAP1 .
	manualset3
96545	6	400116	5	NULL	NULL	0	NULL	effector protein IQGAP1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , activation of PKG inhibits the activity of small GTPase Rac1 and its association with the effector protein IQGAP1 .
	manualset3
96546	1	400117	5	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , all children infected with E. histolytica had serum antibodies to lectin .
	manualset3
96547	2	400117	5	NULL	NULL	0	NULL	 E. histolytica	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , all children infected with E. histolytica had serum antibodies to lectin .
	manualset3
96548	3	400117	5	NULL	NULL	NULL	NULL	serum antibodies	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , all children infected with E. histolytica had serum antibodies to lectin .
	manualset3
96549	4	400117	5	NULL	NULL	0	NULL	lectin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , all children infected with E. histolytica had serum antibodies to lectin .
	manualset3
96550	1	400118	5	NULL	NULL	0	NULL	factor X secretion 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , although factor X secretion was not precluded by warfarin , its gamma-carboxylation was completely blocked .
	manualset3
96551	2	400118	5	NULL	NULL	0	NULL	warfarin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , although factor X secretion was not precluded by warfarin , its gamma-carboxylation was completely blocked .
	manualset3
96552	3	400118	5	NULL	NULL	0	NULL	gamma-carboxylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , although factor X secretion was not precluded by warfarin , its gamma-carboxylation was completely blocked .
	manualset3
96553	1	400119	5	NULL	NULL	0	NULL	 apo-carbonic anhydrase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , apo-carbonic anhydrase abstracts zinc from Zn-thionein and Zn , Cd-thionein in second-order processes that are 2-3 orders of magnitude more rapid than those involving EDTA and approach the rate for unligated Zn2 + with the apo-protein .
	manualset3
96554	2	400119	5	NULL	NULL	NULL	NULL	zinc	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , apo-carbonic anhydrase abstracts zinc from Zn-thionein and Zn , Cd-thionein in second-order processes that are 2-3 orders of magnitude more rapid than those involving EDTA and approach the rate for unligated Zn2 + with the apo-protein .
	manualset3
96555	3	400119	5	NULL	NULL	0	NULL	Zn-thionein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , apo-carbonic anhydrase abstracts zinc from Zn-thionein and Zn , Cd-thionein in second-order processes that are 2-3 orders of magnitude more rapid than those involving EDTA and approach the rate for unligated Zn2 + with the apo-protein .
	manualset3
96556	4	400119	5	NULL	NULL	0	NULL	Zn	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , apo-carbonic anhydrase abstracts zinc from Zn-thionein and Zn , Cd-thionein in second-order processes that are 2-3 orders of magnitude more rapid than those involving EDTA and approach the rate for unligated Zn2 + with the apo-protein .
	manualset3
96557	5	400119	5	NULL	NULL	0	NULL	Cd-thionein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , apo-carbonic anhydrase abstracts zinc from Zn-thionein and Zn , Cd-thionein in second-order processes that are 2-3 orders of magnitude more rapid than those involving EDTA and approach the rate for unligated Zn2 + with the apo-protein .
	manualset3
96558	6	400119	5	NULL	NULL	0	NULL	second-order processes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , apo-carbonic anhydrase abstracts zinc from Zn-thionein and Zn , Cd-thionein in second-order processes that are 2-3 orders of magnitude more rapid than those involving EDTA and approach the rate for unligated Zn2 + with the apo-protein .
	manualset3
96559	7	400119	5	NULL	NULL	0	NULL	2-3 orders of magnitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , apo-carbonic anhydrase abstracts zinc from Zn-thionein and Zn , Cd-thionein in second-order processes that are 2-3 orders of magnitude more rapid than those involving EDTA and approach the rate for unligated Zn2 + with the apo-protein .
	manualset3
96560	8	400119	5	NULL	NULL	0	NULL	EDTA	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , apo-carbonic anhydrase abstracts zinc from Zn-thionein and Zn , Cd-thionein in second-order processes that are 2-3 orders of magnitude more rapid than those involving EDTA and approach the rate for unligated Zn2 + with the apo-protein .
	manualset3
96561	9	400119	5	NULL	NULL	0	NULL	unligated Zn2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , apo-carbonic anhydrase abstracts zinc from Zn-thionein and Zn , Cd-thionein in second-order processes that are 2-3 orders of magnitude more rapid than those involving EDTA and approach the rate for unligated Zn2 + with the apo-protein .
	manualset3
96562	10	400119	5	NULL	NULL	0	NULL	apo-protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , apo-carbonic anhydrase abstracts zinc from Zn-thionein and Zn , Cd-thionein in second-order processes that are 2-3 orders of magnitude more rapid than those involving EDTA and approach the rate for unligated Zn2 + with the apo-protein .
	manualset3
96563	1	400120	5	NULL	NULL	0	NULL	60 % and 20 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , approximately 60 % and 20 % of the MPB CD34 + cells expressed CD33 and c-kit antigens , respectively .
	manualset3
96564	2	400120	5	NULL	NULL	0	NULL	MPB CD34 + cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , approximately 60 % and 20 % of the MPB CD34 + cells expressed CD33 and c-kit antigens , respectively .
	manualset3
96565	3	400120	5	NULL	NULL	0	NULL	CD33	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , approximately 60 % and 20 % of the MPB CD34 + cells expressed CD33 and c-kit antigens , respectively .
	manualset3
96566	4	400120	5	NULL	NULL	0	NULL	c-kit antigens	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , approximately 60 % and 20 % of the MPB CD34 + cells expressed CD33 and c-kit antigens , respectively .
	manualset3
96567	1	400121	5	NULL	NULL	0	NULL	bilateral peripheral vestibular lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , bilateral peripheral vestibular lesions altered the pattern of orthostatic responses in all animals , and blood pressure fluctuated ) 10 mmHg from baseline values during most 60 degrees nose-up tilts in five of six animals .
	manualset3
96568	2	400121	5	NULL	NULL	0	NULL	pattern	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , bilateral peripheral vestibular lesions altered the pattern of orthostatic responses in all animals , and blood pressure fluctuated ) 10 mmHg from baseline values during most 60 degrees nose-up tilts in five of six animals .
	manualset3
96569	3	400121	5	NULL	NULL	0	NULL	orthostatic responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , bilateral peripheral vestibular lesions altered the pattern of orthostatic responses in all animals , and blood pressure fluctuated ) 10 mmHg from baseline values during most 60 degrees nose-up tilts in five of six animals .
	manualset3
96570	4	400121	5	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , bilateral peripheral vestibular lesions altered the pattern of orthostatic responses in all animals , and blood pressure fluctuated ) 10 mmHg from baseline values during most 60 degrees nose-up tilts in five of six animals .
	manualset3
96571	5	400121	5	NULL	NULL	0	NULL	blood pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , bilateral peripheral vestibular lesions altered the pattern of orthostatic responses in all animals , and blood pressure fluctuated ) 10 mmHg from baseline values during most 60 degrees nose-up tilts in five of six animals .
	manualset3
96572	6	400121	5	NULL	NULL	0	NULL	10 mmHg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , bilateral peripheral vestibular lesions altered the pattern of orthostatic responses in all animals , and blood pressure fluctuated ) 10 mmHg from baseline values during most 60 degrees nose-up tilts in five of six animals .
	manualset3
96573	7	400121	5	NULL	NULL	0	NULL	baseline values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , bilateral peripheral vestibular lesions altered the pattern of orthostatic responses in all animals , and blood pressure fluctuated ) 10 mmHg from baseline values during most 60 degrees nose-up tilts in five of six animals .
	manualset3
96574	8	400121	5	NULL	NULL	0	NULL	60 degrees nose-up tilts 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , bilateral peripheral vestibular lesions altered the pattern of orthostatic responses in all animals , and blood pressure fluctuated ) 10 mmHg from baseline values during most 60 degrees nose-up tilts in five of six animals .
	manualset3
96575	9	400121	5	NULL	NULL	0	NULL	five of six animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , bilateral peripheral vestibular lesions altered the pattern of orthostatic responses in all animals , and blood pressure fluctuated ) 10 mmHg from baseline values during most 60 degrees nose-up tilts in five of six animals .
	manualset3
96576	1	400122	5	NULL	NULL	0	NULL	calcium ionophore A23187	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , calcium ionophore A23187 elicited a single peak of early PAF synthesis .
	manualset3
96577	2	400122	5	NULL	NULL	0	NULL	single peak	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , calcium ionophore A23187 elicited a single peak of early PAF synthesis .
	manualset3
96578	3	400122	5	NULL	NULL	0	NULL	early PAF synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , calcium ionophore A23187 elicited a single peak of early PAF synthesis .
	manualset3
96579	1	400123	5	NULL	NULL	0	NULL	competition experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , competition experiments using gel shift assays suggest that RAGE interaction with AGE is driven by the recognition of negative charges on AGE-proteins .
	manualset3
96580	2	400123	5	NULL	NULL	0	NULL	gel shift assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , competition experiments using gel shift assays suggest that RAGE interaction with AGE is driven by the recognition of negative charges on AGE-proteins .
	manualset3
96581	3	400123	5	NULL	NULL	0	NULL	RAGE interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , competition experiments using gel shift assays suggest that RAGE interaction with AGE is driven by the recognition of negative charges on AGE-proteins .
	manualset3
96582	4	400123	5	NULL	NULL	0	NULL	AGE	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , competition experiments using gel shift assays suggest that RAGE interaction with AGE is driven by the recognition of negative charges on AGE-proteins .
	manualset3
96583	5	400123	5	NULL	NULL	0	NULL	recognition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , competition experiments using gel shift assays suggest that RAGE interaction with AGE is driven by the recognition of negative charges on AGE-proteins .
	manualset3
96584	6	400123	5	NULL	NULL	0	NULL	AGE-proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , competition experiments using gel shift assays suggest that RAGE interaction with AGE is driven by the recognition of negative charges on AGE-proteins .
	manualset3
96585	1	400124	5	NULL	NULL	0	NULL	professional status	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	( We introduce : the professional status of speech therapists and their contribution to `` the right to speech '' ) .
	manualset3
96586	2	400124	5	NULL	NULL	0	NULL	speech therapists 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( We introduce : the professional status of speech therapists and their contribution to `` the right to speech '' ) .
	manualset3
96587	3	400124	5	NULL	NULL	0	NULL	contribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( We introduce : the professional status of speech therapists and their contribution to `` the right to speech '' ) .
	manualset3
96588	4	400124	5	NULL	NULL	0	NULL	speech	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( We introduce : the professional status of speech therapists and their contribution to `` the right to speech '' ) .
	manualset3
96589	1	400125	5	NULL	NULL	0	NULL	deletion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , deletion of the 13 amino acid long C-terminal region of eIF-2 alpha , including the three phosphorylation sites , led to derepression of GCN4 in vivo .
	manualset3
96590	2	400125	5	NULL	NULL	0	NULL	13 amino acid long C-terminal region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , deletion of the 13 amino acid long C-terminal region of eIF-2 alpha , including the three phosphorylation sites , led to derepression of GCN4 in vivo .
	manualset3
96591	3	400125	5	NULL	NULL	0	NULL	eIF-2 alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , deletion of the 13 amino acid long C-terminal region of eIF-2 alpha , including the three phosphorylation sites , led to derepression of GCN4 in vivo .
	manualset3
96592	4	400125	5	NULL	NULL	0	NULL	phosphorylation sites	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , deletion of the 13 amino acid long C-terminal region of eIF-2 alpha , including the three phosphorylation sites , led to derepression of GCN4 in vivo .
	manualset3
96593	5	400125	5	NULL	NULL	0	NULL	derepression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , deletion of the 13 amino acid long C-terminal region of eIF-2 alpha , including the three phosphorylation sites , led to derepression of GCN4 in vivo .
	manualset3
96594	6	400125	5	NULL	NULL	0	NULL	GCN4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , deletion of the 13 amino acid long C-terminal region of eIF-2 alpha , including the three phosphorylation sites , led to derepression of GCN4 in vivo .
	manualset3
96595	1	400126	5	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , evidence to date suggests that visuomotor learning does not consolidate .
	manualset3
96596	2	400126	5	NULL	NULL	0	NULL	to date	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , evidence to date suggests that visuomotor learning does not consolidate .
	manualset3
96598	3	400126	5	NULL	NULL	0	NULL	visuomotor learning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , evidence to date suggests that visuomotor learning does not consolidate .
	manualset3
96600	1	400127	5	NULL	NULL	0	NULL	experimental data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , experimental data provide evidence for a non-uniform alveolar region coupled with sequential filling of the lung .
	manualset3
96602	2	400127	5	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , experimental data provide evidence for a non-uniform alveolar region coupled with sequential filling of the lung .
	manualset3
96604	3	400127	5	NULL	NULL	NULL	NULL	non-uniform alveolar region	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , experimental data provide evidence for a non-uniform alveolar region coupled with sequential filling of the lung .
	manualset3
96610	4	400127	5	NULL	NULL	0	NULL	sequential filling of the lung	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , experimental data provide evidence for a non-uniform alveolar region coupled with sequential filling of the lung .
	manualset3
96611	1	400128	5	NULL	NULL	0	NULL	experimental human studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , experimental human studies of local arterial inflammation , such as the brachial artery infusion of TNF-alpha ( tumor necrosis factor-alpha ) model reported in this issue of Clinical Science by Robinson and co-workers , are of value in elucidating the pathophysiology of atherothrombosis .
	manualset3
96612	2	400128	5	NULL	NULL	0	NULL	local arterial inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , experimental human studies of local arterial inflammation , such as the brachial artery infusion of TNF-alpha ( tumor necrosis factor-alpha ) model reported in this issue of Clinical Science by Robinson and co-workers , are of value in elucidating the pathophysiology of atherothrombosis .
	manualset3
96613	3	400128	5	NULL	NULL	NULL	NULL	 brachial artery infusion of TNF-alpha ( tumor necrosis factor-alpha ) model 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , experimental human studies of local arterial inflammation , such as the brachial artery infusion of TNF-alpha ( tumor necrosis factor-alpha ) model reported in this issue of Clinical Science by Robinson and co-workers , are of value in elucidating the pathophysiology of atherothrombosis .
	manualset3
96614	4	400128	5	NULL	NULL	0	NULL	issue of Clinical Science	Journal												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , experimental human studies of local arterial inflammation , such as the brachial artery infusion of TNF-alpha ( tumor necrosis factor-alpha ) model reported in this issue of Clinical Science by Robinson and co-workers , are of value in elucidating the pathophysiology of atherothrombosis .
	manualset3
96615	5	400128	5	NULL	NULL	0	NULL	Robinson	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , experimental human studies of local arterial inflammation , such as the brachial artery infusion of TNF-alpha ( tumor necrosis factor-alpha ) model reported in this issue of Clinical Science by Robinson and co-workers , are of value in elucidating the pathophysiology of atherothrombosis .
	manualset3
96616	6	400128	5	NULL	NULL	0	NULL	co-workers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , experimental human studies of local arterial inflammation , such as the brachial artery infusion of TNF-alpha ( tumor necrosis factor-alpha ) model reported in this issue of Clinical Science by Robinson and co-workers , are of value in elucidating the pathophysiology of atherothrombosis .
	manualset3
96617	7	400128	5	NULL	NULL	0	NULL	value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , experimental human studies of local arterial inflammation , such as the brachial artery infusion of TNF-alpha ( tumor necrosis factor-alpha ) model reported in this issue of Clinical Science by Robinson and co-workers , are of value in elucidating the pathophysiology of atherothrombosis .
	manualset3
96618	8	400128	5	NULL	NULL	0	NULL	pathophysiology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , experimental human studies of local arterial inflammation , such as the brachial artery infusion of TNF-alpha ( tumor necrosis factor-alpha ) model reported in this issue of Clinical Science by Robinson and co-workers , are of value in elucidating the pathophysiology of atherothrombosis .
	manualset3
96619	9	400128	5	NULL	NULL	0	NULL	atherothrombosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , experimental human studies of local arterial inflammation , such as the brachial artery infusion of TNF-alpha ( tumor necrosis factor-alpha ) model reported in this issue of Clinical Science by Robinson and co-workers , are of value in elucidating the pathophysiology of atherothrombosis .
	manualset3
96620	1	400129	5	NULL	NULL	NULL	NULL	expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , expression of the short HOXA10 transcript , HOXA10b , was almost exclusively found in the TCRbeta-HOXA rearranged cases , suggesting a specific role for the HOXA10b short transcript in TCRbeta-HOXA-mediated oncogenesis .
	manualset3
96621	2	400129	5	NULL	NULL	NULL	NULL	short HOXA10 transcript , HOXA10b	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , expression of the short HOXA10 transcript , HOXA10b , was almost exclusively found in the TCRbeta-HOXA rearranged cases , suggesting a specific role for the HOXA10b short transcript in TCRbeta-HOXA-mediated oncogenesis .
	manualset3
96623	3	400129	5	NULL	NULL	NULL	NULL	TCRbeta-HOXA rearranged cases	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , expression of the short HOXA10 transcript , HOXA10b , was almost exclusively found in the TCRbeta-HOXA rearranged cases , suggesting a specific role for the HOXA10b short transcript in TCRbeta-HOXA-mediated oncogenesis .
	manualset3
96624	4	400129	5	NULL	NULL	NULL	NULL	specific role 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , expression of the short HOXA10 transcript , HOXA10b , was almost exclusively found in the TCRbeta-HOXA rearranged cases , suggesting a specific role for the HOXA10b short transcript in TCRbeta-HOXA-mediated oncogenesis .
	manualset3
96625	5	400129	5	NULL	NULL	NULL	NULL	HOXA10b short transcript	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , expression of the short HOXA10 transcript , HOXA10b , was almost exclusively found in the TCRbeta-HOXA rearranged cases , suggesting a specific role for the HOXA10b short transcript in TCRbeta-HOXA-mediated oncogenesis .
	manualset3
96626	6	400129	5	NULL	NULL	NULL	NULL	TCRbeta-HOXA-mediated oncogenesis	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , expression of the short HOXA10 transcript , HOXA10b , was almost exclusively found in the TCRbeta-HOXA rearranged cases , suggesting a specific role for the HOXA10b short transcript in TCRbeta-HOXA-mediated oncogenesis .
	manualset3
96627	1	400130	5	NULL	NULL	NULL	NULL	expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , expression of xylE in urea or picB decreased after parallel exposure to acid pH ( pH 7 ) 6 ) 5 ) 4 ) , regardless of the growth phase .
	manualset3
96628	2	400130	5	NULL	NULL	0	NULL	xylE	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , expression of xylE in urea or picB decreased after parallel exposure to acid pH ( pH 7 ) 6 ) 5 ) 4 ) , regardless of the growth phase .
	manualset3
96629	3	400130	5	NULL	NULL	0	NULL	urea	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , expression of xylE in urea or picB decreased after parallel exposure to acid pH ( pH 7 ) 6 ) 5 ) 4 ) , regardless of the growth phase .
	manualset3
96630	4	400130	5	NULL	NULL	0	NULL	picB	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , expression of xylE in urea or picB decreased after parallel exposure to acid pH ( pH 7 ) 6 ) 5 ) 4 ) , regardless of the growth phase .
	manualset3
96631	5	400130	5	NULL	NULL	0	NULL	parallel exposure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , expression of xylE in urea or picB decreased after parallel exposure to acid pH ( pH 7 ) 6 ) 5 ) 4 ) , regardless of the growth phase .
	manualset3
96632	6	400130	5	NULL	NULL	0	NULL	acid pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , expression of xylE in urea or picB decreased after parallel exposure to acid pH ( pH 7 ) 6 ) 5 ) 4 ) , regardless of the growth phase .
	manualset3
96633	7	400130	5	NULL	NULL	0	NULL	( pH 7 ) 6 ) 5 ) 4 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , expression of xylE in urea or picB decreased after parallel exposure to acid pH ( pH 7 ) 6 ) 5 ) 4 ) , regardless of the growth phase .
	manualset3
96634	8	400130	5	NULL	NULL	NULL	NULL	growth phase	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , expression of xylE in urea or picB decreased after parallel exposure to acid pH ( pH 7 ) 6 ) 5 ) 4 ) , regardless of the growth phase .
	manualset3
97111	1	400131	5	NULL	NULL	0	NULL	high-dose trials	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , high-dose trials performed in conjunction with autologous hematopoietic stem cell transplantation have demonstrated objective responses in 95 % of patients , complete responses in 85 % of patients , with a progression-free survival of 62 % and an overall survival of 93 % with a median follow-up of two years .
	manualset3
97112	2	400131	5	NULL	NULL	0	NULL	conjunction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , high-dose trials performed in conjunction with autologous hematopoietic stem cell transplantation have demonstrated objective responses in 95 % of patients , complete responses in 85 % of patients , with a progression-free survival of 62 % and an overall survival of 93 % with a median follow-up of two years .
	manualset3
97113	3	400131	5	NULL	NULL	0	NULL	autologous hematopoietic stem cell transplantation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , high-dose trials performed in conjunction with autologous hematopoietic stem cell transplantation have demonstrated objective responses in 95 % of patients , complete responses in 85 % of patients , with a progression-free survival of 62 % and an overall survival of 93 % with a median follow-up of two years .
	manualset3
97114	4	400131	5	NULL	NULL	NULL	NULL	objective responses 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , high-dose trials performed in conjunction with autologous hematopoietic stem cell transplantation have demonstrated objective responses in 95 % of patients , complete responses in 85 % of patients , with a progression-free survival of 62 % and an overall survival of 93 % with a median follow-up of two years .
	manualset3
97115	5	400131	5	NULL	NULL	0	NULL	 95 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , high-dose trials performed in conjunction with autologous hematopoietic stem cell transplantation have demonstrated objective responses in 95 % of patients , complete responses in 85 % of patients , with a progression-free survival of 62 % and an overall survival of 93 % with a median follow-up of two years .
	manualset3
97116	6	400131	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , high-dose trials performed in conjunction with autologous hematopoietic stem cell transplantation have demonstrated objective responses in 95 % of patients , complete responses in 85 % of patients , with a progression-free survival of 62 % and an overall survival of 93 % with a median follow-up of two years .
	manualset3
97117	7	400131	5	NULL	NULL	NULL	NULL	complete responses	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , high-dose trials performed in conjunction with autologous hematopoietic stem cell transplantation have demonstrated objective responses in 95 % of patients , complete responses in 85 % of patients , with a progression-free survival of 62 % and an overall survival of 93 % with a median follow-up of two years .
	manualset3
97118	8	400131	5	NULL	NULL	0	NULL	85 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , high-dose trials performed in conjunction with autologous hematopoietic stem cell transplantation have demonstrated objective responses in 95 % of patients , complete responses in 85 % of patients , with a progression-free survival of 62 % and an overall survival of 93 % with a median follow-up of two years .
	manualset3
97119	9	400131	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , high-dose trials performed in conjunction with autologous hematopoietic stem cell transplantation have demonstrated objective responses in 95 % of patients , complete responses in 85 % of patients , with a progression-free survival of 62 % and an overall survival of 93 % with a median follow-up of two years .
	manualset3
97120	10	400131	5	NULL	NULL	NULL	NULL	progression-free survival 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , high-dose trials performed in conjunction with autologous hematopoietic stem cell transplantation have demonstrated objective responses in 95 % of patients , complete responses in 85 % of patients , with a progression-free survival of 62 % and an overall survival of 93 % with a median follow-up of two years .
	manualset3
97121	11	400131	5	NULL	NULL	0	NULL	62 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , high-dose trials performed in conjunction with autologous hematopoietic stem cell transplantation have demonstrated objective responses in 95 % of patients , complete responses in 85 % of patients , with a progression-free survival of 62 % and an overall survival of 93 % with a median follow-up of two years .
	manualset3
97122	12	400131	5	NULL	NULL	NULL	NULL	survival	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , high-dose trials performed in conjunction with autologous hematopoietic stem cell transplantation have demonstrated objective responses in 95 % of patients , complete responses in 85 % of patients , with a progression-free survival of 62 % and an overall survival of 93 % with a median follow-up of two years .
	manualset3
97123	13	400131	5	NULL	NULL	0	NULL	93 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , high-dose trials performed in conjunction with autologous hematopoietic stem cell transplantation have demonstrated objective responses in 95 % of patients , complete responses in 85 % of patients , with a progression-free survival of 62 % and an overall survival of 93 % with a median follow-up of two years .
	manualset3
97124	14	400131	5	NULL	NULL	0	NULL	two years	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , high-dose trials performed in conjunction with autologous hematopoietic stem cell transplantation have demonstrated objective responses in 95 % of patients , complete responses in 85 % of patients , with a progression-free survival of 62 % and an overall survival of 93 % with a median follow-up of two years .
	manualset3
97125	1	400132	5	NULL	NULL	0	NULL	subset of rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , in a subset of rats ( n = 35 ) with reduced renal mass but intact parathyroid glands similarly treated with the vitamin D metabolites , a blunted calcemic response was seen after the combination of 1 , 25 ( OH ) 2D3 with 25 , 25 ( OH ) 2D3 administration alone .
	manualset3
97126	2	400132	5	NULL	NULL	0	NULL	n = 35	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , in a subset of rats ( n = 35 ) with reduced renal mass but intact parathyroid glands similarly treated with the vitamin D metabolites , a blunted calcemic response was seen after the combination of 1 , 25 ( OH ) 2D3 with 25 , 25 ( OH ) 2D3 administration alone .
	manualset3
97127	3	400132	5	NULL	NULL	NULL	NULL	reduced renal mass	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , in a subset of rats ( n = 35 ) with reduced renal mass but intact parathyroid glands similarly treated with the vitamin D metabolites , a blunted calcemic response was seen after the combination of 1 , 25 ( OH ) 2D3 with 25 , 25 ( OH ) 2D3 administration alone .
	manualset3
97128	4	400132	5	NULL	NULL	0	NULL	intact parathyroid glands	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , in a subset of rats ( n = 35 ) with reduced renal mass but intact parathyroid glands similarly treated with the vitamin D metabolites , a blunted calcemic response was seen after the combination of 1 , 25 ( OH ) 2D3 with 25 , 25 ( OH ) 2D3 administration alone .
	manualset3
97134	5	400132	5	NULL	NULL	0	NULL	vitamin D metabolites	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , in a subset of rats ( n = 35 ) with reduced renal mass but intact parathyroid glands similarly treated with the vitamin D metabolites , a blunted calcemic response was seen after the combination of 1 , 25 ( OH ) 2D3 with 25 , 25 ( OH ) 2D3 administration alone .
	manualset3
97135	6	400132	5	NULL	NULL	NULL	NULL	blunted calcemic response	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , in a subset of rats ( n = 35 ) with reduced renal mass but intact parathyroid glands similarly treated with the vitamin D metabolites , a blunted calcemic response was seen after the combination of 1 , 25 ( OH ) 2D3 with 25 , 25 ( OH ) 2D3 administration alone .
	manualset3
97136	7	400132	5	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , in a subset of rats ( n = 35 ) with reduced renal mass but intact parathyroid glands similarly treated with the vitamin D metabolites , a blunted calcemic response was seen after the combination of 1 , 25 ( OH ) 2D3 with 25 , 25 ( OH ) 2D3 administration alone .
	manualset3
97137	8	400132	5	NULL	NULL	0	NULL	1 , 25 ( OH ) 2D3	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , in a subset of rats ( n = 35 ) with reduced renal mass but intact parathyroid glands similarly treated with the vitamin D metabolites , a blunted calcemic response was seen after the combination of 1 , 25 ( OH ) 2D3 with 25 , 25 ( OH ) 2D3 administration alone .
	manualset3
97138	9	400132	5	NULL	NULL	0	NULL	25 , 25 ( OH ) 2D3 administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , in a subset of rats ( n = 35 ) with reduced renal mass but intact parathyroid glands similarly treated with the vitamin D metabolites , a blunted calcemic response was seen after the combination of 1 , 25 ( OH ) 2D3 with 25 , 25 ( OH ) 2D3 administration alone .
	manualset3
97139	1	400133	5	NULL	NULL	0	NULL	advantages	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	( What are the advantages of magnetic resonance tomography compared with computerized tomography in imaging spontaneous cerebral hemorrhage ? ) .
	manualset3
97142	2	400133	5	NULL	NULL	0	NULL	magnetic resonance tomography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( What are the advantages of magnetic resonance tomography compared with computerized tomography in imaging spontaneous cerebral hemorrhage ? ) .
	manualset3
97143	3	400133	5	NULL	NULL	0	NULL	computerized tomography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( What are the advantages of magnetic resonance tomography compared with computerized tomography in imaging spontaneous cerebral hemorrhage ? ) .
	manualset3
97145	4	400133	5	NULL	NULL	0	NULL	spontaneous cerebral hemorrhage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( What are the advantages of magnetic resonance tomography compared with computerized tomography in imaging spontaneous cerebral hemorrhage ? ) .
	manualset3
97146	1	400134	5	NULL	NULL	0	NULL	hypothyroidism	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , in hypothyroidism hepatic glutathione may be increased and thus renders the liver less sensitive to alcohol generated free radical production .
	manualset3
97147	2	400134	5	NULL	NULL	0	NULL	hepatic glutathione	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , in hypothyroidism hepatic glutathione may be increased and thus renders the liver less sensitive to alcohol generated free radical production .
	manualset3
97148	3	400134	5	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , in hypothyroidism hepatic glutathione may be increased and thus renders the liver less sensitive to alcohol generated free radical production .
	manualset3
97149	4	400134	5	NULL	NULL	NULL	NULL	alcohol	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , in hypothyroidism hepatic glutathione may be increased and thus renders the liver less sensitive to alcohol generated free radical production .
	manualset3
97150	5	400134	5	NULL	NULL	0	NULL	free radical production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , in hypothyroidism hepatic glutathione may be increased and thus renders the liver less sensitive to alcohol generated free radical production .
	manualset3
97151	1	400135	5	NULL	NULL	0	NULL	infusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , infusion of high-dose sufentanil ( group 3 ) was associated with 27 to 30 % decreases in CBFV ( p & lt ; 0.05 ) .
	manualset3
97152	2	400135	5	NULL	NULL	0	NULL	high-dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , infusion of high-dose sufentanil ( group 3 ) was associated with 27 to 30 % decreases in CBFV ( p & lt ; 0.05 ) .
	manualset3
97153	3	400135	5	NULL	NULL	0	NULL	sufentanil ( group 3 )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , infusion of high-dose sufentanil ( group 3 ) was associated with 27 to 30 % decreases in CBFV ( p & lt ; 0.05 ) .
	manualset3
97154	4	400135	5	NULL	NULL	0	NULL	 27 to 30 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , infusion of high-dose sufentanil ( group 3 ) was associated with 27 to 30 % decreases in CBFV ( p & lt ; 0.05 ) .
	manualset3
97155	5	400135	5	NULL	NULL	0	NULL	CBFV	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , infusion of high-dose sufentanil ( group 3 ) was associated with 27 to 30 % decreases in CBFV ( p & lt ; 0.05 ) .
	manualset3
97156	6	400135	5	NULL	NULL	0	NULL	p & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , infusion of high-dose sufentanil ( group 3 ) was associated with 27 to 30 % decreases in CBFV ( p & lt ; 0.05 ) .
	manualset3
97157	1	400136	5	NULL	NULL	0	NULL	inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , inhibition of ROCK by Y27632 neither altered the actin stress fibers nor induced chondrogenesis .
	manualset3
97158	2	400136	5	NULL	NULL	0	NULL	ROCK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , inhibition of ROCK by Y27632 neither altered the actin stress fibers nor induced chondrogenesis .
	manualset3
97159	3	400136	5	NULL	NULL	0	NULL	Y27632	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , inhibition of ROCK by Y27632 neither altered the actin stress fibers nor induced chondrogenesis .
	manualset3
97160	4	400136	5	NULL	NULL	0	NULL	actin stress fibers	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , inhibition of ROCK by Y27632 neither altered the actin stress fibers nor induced chondrogenesis .
	manualset3
97161	5	400136	5	NULL	NULL	0	NULL	chondrogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , inhibition of ROCK by Y27632 neither altered the actin stress fibers nor induced chondrogenesis .
	manualset3
97162	1	400137	5	NULL	NULL	0	NULL	inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , inhibition of protein kinase C ( PKC ) by chelerythrine did not affect KCl - or PE-induced contractions , indicating lack of participation of PKC-mediated Ca2 + sensitization .
	manualset3
97163	2	400137	5	NULL	NULL	0	NULL	 protein kinase C ( PKC )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , inhibition of protein kinase C ( PKC ) by chelerythrine did not affect KCl - or PE-induced contractions , indicating lack of participation of PKC-mediated Ca2 + sensitization .
	manualset3
97164	3	400137	5	NULL	NULL	0	NULL	chelerythrine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , inhibition of protein kinase C ( PKC ) by chelerythrine did not affect KCl - or PE-induced contractions , indicating lack of participation of PKC-mediated Ca2 + sensitization .
	manualset3
97165	4	400137	5	NULL	NULL	0	NULL	KCl - or PE-induced contractions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , inhibition of protein kinase C ( PKC ) by chelerythrine did not affect KCl - or PE-induced contractions , indicating lack of participation of PKC-mediated Ca2 + sensitization .
	manualset3
97166	5	400137	5	NULL	NULL	0	NULL	participation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , inhibition of protein kinase C ( PKC ) by chelerythrine did not affect KCl - or PE-induced contractions , indicating lack of participation of PKC-mediated Ca2 + sensitization .
	manualset3
97167	6	400137	5	NULL	NULL	0	NULL	PKC-mediated Ca2 + sensitization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , inhibition of protein kinase C ( PKC ) by chelerythrine did not affect KCl - or PE-induced contractions , indicating lack of participation of PKC-mediated Ca2 + sensitization .
	manualset3
97168	1	400138	5	NULL	NULL	0	NULL	interleukin-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , interleukin-1 was not cytotoxic to HUVEC , nor did it enhance cell death in combination with Shiga toxin .
	manualset3
97170	2	400138	5	NULL	NULL	NULL	NULL	HUVEC	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , interleukin-1 was not cytotoxic to HUVEC , nor did it enhance cell death in combination with Shiga toxin .
	manualset3
97171	3	400138	5	NULL	NULL	NULL	NULL	cell death	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , interleukin-1 was not cytotoxic to HUVEC , nor did it enhance cell death in combination with Shiga toxin .
	manualset3
97172	4	400138	5	NULL	NULL	NULL	NULL	combination	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , interleukin-1 was not cytotoxic to HUVEC , nor did it enhance cell death in combination with Shiga toxin .
	manualset3
97173	5	400138	5	NULL	NULL	NULL	NULL	Shiga toxin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , interleukin-1 was not cytotoxic to HUVEC , nor did it enhance cell death in combination with Shiga toxin .
	manualset3
97174	1	400139	5	NULL	NULL	0	NULL	pelvic girdle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , its pelvic girdle and hind limb have no aquatic modifications .
	manualset3
97175	2	400139	5	NULL	NULL	0	NULL	hind limb	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , its pelvic girdle and hind limb have no aquatic modifications .
	manualset3
97176	3	400139	5	NULL	NULL	0	NULL	aquatic modifications	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , its pelvic girdle and hind limb have no aquatic modifications .
	manualset3
97177	1	400140	5	NULL	NULL	0	NULL	general principles	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	( What are the general principles and management of patients presenting with respiratory diseases and preparing for air travel ?
	manualset3
97178	2	400140	5	NULL	NULL	0	NULL	management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( What are the general principles and management of patients presenting with respiratory diseases and preparing for air travel ?
	manualset3
97179	3	400140	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( What are the general principles and management of patients presenting with respiratory diseases and preparing for air travel ?
	manualset3
97180	4	400140	5	NULL	NULL	0	NULL	respiratory diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( What are the general principles and management of patients presenting with respiratory diseases and preparing for air travel ?
	manualset3
97181	5	400140	5	NULL	NULL	0	NULL	air travel	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( What are the general principles and management of patients presenting with respiratory diseases and preparing for air travel ?
	manualset3
97182	1	400141	5	NULL	NULL	0	NULL	opposite process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , little is known about the opposite process , when the amount of habitat decreases .
	manualset3
97183	2	400141	5	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , little is known about the opposite process , when the amount of habitat decreases .
	manualset3
97184	3	400141	5	NULL	NULL	0	NULL	habitat	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , little is known about the opposite process , when the amount of habitat decreases .
	manualset3
97185	1	400142	5	NULL	NULL	0	NULL	marrow implants	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , marrow implants from patients in the chronic phase of CML ( six patients ) showed infrequent and limited myeloid growth in the mice .
	manualset3
97186	2	400142	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , marrow implants from patients in the chronic phase of CML ( six patients ) showed infrequent and limited myeloid growth in the mice .
	manualset3
97187	3	400142	5	NULL	NULL	0	NULL	chronic phase of CML	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , marrow implants from patients in the chronic phase of CML ( six patients ) showed infrequent and limited myeloid growth in the mice .
	manualset3
97188	4	400142	5	NULL	NULL	0	NULL	six patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , marrow implants from patients in the chronic phase of CML ( six patients ) showed infrequent and limited myeloid growth in the mice .
	manualset3
97189	5	400142	5	NULL	NULL	0	NULL	infrequent and limited myeloid growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , marrow implants from patients in the chronic phase of CML ( six patients ) showed infrequent and limited myeloid growth in the mice .
	manualset3
97190	6	400142	5	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , marrow implants from patients in the chronic phase of CML ( six patients ) showed infrequent and limited myeloid growth in the mice .
	manualset3
97191	1	400143	5	NULL	NULL	0	NULL	mid-infrared spectra	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , mid-infrared spectra are presented that qualitatively demonstrate the rapid rate at which atmospheric moisture is incorporated into the anhydrous sample when analyzed using the conventional ATR cell assembly .
	manualset3
97193	2	400143	5	NULL	NULL	NULL	NULL	rapid rate	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , mid-infrared spectra are presented that qualitatively demonstrate the rapid rate at which atmospheric moisture is incorporated into the anhydrous sample when analyzed using the conventional ATR cell assembly .
	manualset3
97194	3	400143	5	NULL	NULL	NULL	NULL	atmospheric moisture	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , mid-infrared spectra are presented that qualitatively demonstrate the rapid rate at which atmospheric moisture is incorporated into the anhydrous sample when analyzed using the conventional ATR cell assembly .
	manualset3
97196	4	400143	5	NULL	NULL	NULL	NULL	anhydrous sample	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , mid-infrared spectra are presented that qualitatively demonstrate the rapid rate at which atmospheric moisture is incorporated into the anhydrous sample when analyzed using the conventional ATR cell assembly .
	manualset3
97198	5	400143	5	NULL	NULL	NULL	NULL	conventional ATR cell assembly	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , mid-infrared spectra are presented that qualitatively demonstrate the rapid rate at which atmospheric moisture is incorporated into the anhydrous sample when analyzed using the conventional ATR cell assembly .
	manualset3
97200	1	400144	5	NULL	NULL	NULL	NULL	wild-type Rab10	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , neither wild-type nor constitutively active GFP-tagged Rab10 restored GLUT4 translocation .
	manualset3
97201	2	400144	5	NULL	NULL	0	NULL	constitutively active GFP-tagged Rab10	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , neither wild-type nor constitutively active GFP-tagged Rab10 restored GLUT4 translocation .
	manualset3
97203	3	400144	5	NULL	NULL	0	NULL	GLUT4 translocation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , neither wild-type nor constitutively active GFP-tagged Rab10 restored GLUT4 translocation .
	manualset3
97205	1	400145	5	NULL	NULL	0	NULL	net backflux	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , net backflux of calcium was negligible .
	manualset3
97207	2	400145	5	NULL	NULL	0	NULL	calcium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , net backflux of calcium was negligible .
	manualset3
97209	1	400146	5	NULL	NULL	0	NULL	neurites	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , neurites of mutant neurons were markedly resistant to vinblastine-induced degeneration , and both the MMP and the ATP content in the neurites were well maintained .
	manualset3
97210	2	400146	5	NULL	NULL	0	NULL	mutant neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , neurites of mutant neurons were markedly resistant to vinblastine-induced degeneration , and both the MMP and the ATP content in the neurites were well maintained .
	manualset3
97211	3	400146	5	NULL	NULL	0	NULL	vinblastine-induced degeneration	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , neurites of mutant neurons were markedly resistant to vinblastine-induced degeneration , and both the MMP and the ATP content in the neurites were well maintained .
	manualset3
97212	4	400146	5	NULL	NULL	NULL	NULL	MMP content	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , neurites of mutant neurons were markedly resistant to vinblastine-induced degeneration , and both the MMP and the ATP content in the neurites were well maintained .
	manualset3
97213	5	400146	5	NULL	NULL	0	NULL	ATP content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , neurites of mutant neurons were markedly resistant to vinblastine-induced degeneration , and both the MMP and the ATP content in the neurites were well maintained .
	manualset3
97214	6	400146	5	NULL	NULL	0	NULL	neurites	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , neurites of mutant neurons were markedly resistant to vinblastine-induced degeneration , and both the MMP and the ATP content in the neurites were well maintained .
	manualset3
97215	1	400147	5	NULL	NULL	0	NULL	ANAS spent medium	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , only ANAS spent medium resulted in the downregulation of three duplicated genes ( DET0657-0659 / DET0691-0693 ) encoded downstream of a second putative cobalamin riboswitch .
	manualset3
97216	2	400147	5	NULL	NULL	0	NULL	downregulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , only ANAS spent medium resulted in the downregulation of three duplicated genes ( DET0657-0659 / DET0691-0693 ) encoded downstream of a second putative cobalamin riboswitch .
	manualset3
97217	3	400147	5	NULL	NULL	0	NULL	duplicated genes ( DET0657-0659 / DET0691-0693 )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , only ANAS spent medium resulted in the downregulation of three duplicated genes ( DET0657-0659 / DET0691-0693 ) encoded downstream of a second putative cobalamin riboswitch .
	manualset3
97218	4	400147	5	NULL	NULL	0	NULL	second putative cobalamin riboswitch	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , only ANAS spent medium resulted in the downregulation of three duplicated genes ( DET0657-0659 / DET0691-0693 ) encoded downstream of a second putative cobalamin riboswitch .
	manualset3
97219	1	400148	5	NULL	NULL	0	NULL	emotionality	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( What do we have against emotionality ? ) .
	manualset3
97220	1	400149	5	NULL	NULL	0	NULL	direct/ipsilateral AKI group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , only the direct/ipsilateral AKI group demonstrated significant CKD following exposure to elevated salt .
	manualset3
97221	2	400149	5	NULL	NULL	0	NULL	significant CKD 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , only the direct/ipsilateral AKI group demonstrated significant CKD following exposure to elevated salt .
	manualset3
97222	3	400149	5	NULL	NULL	0	NULL	exposure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , only the direct/ipsilateral AKI group demonstrated significant CKD following exposure to elevated salt .
	manualset3
97223	4	400149	5	NULL	NULL	0	NULL	elevated salt	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , only the direct/ipsilateral AKI group demonstrated significant CKD following exposure to elevated salt .
	manualset3
97224	1	400150	5	NULL	NULL	NULL	NULL	K + channel inhibitors ( 4-aminopyridine and tetraethylammonium )	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , other K + channel inhibitors ( 4-aminopyridine and tetraethylammonium ) , at concentrations without marked effects on K ( ir ) , failed to affect neurite extension .
	manualset3
97225	2	400150	5	NULL	NULL	0	NULL	concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , other K + channel inhibitors ( 4-aminopyridine and tetraethylammonium ) , at concentrations without marked effects on K ( ir ) , failed to affect neurite extension .
	manualset3
97226	3	400150	5	NULL	NULL	0	NULL	marked effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , other K + channel inhibitors ( 4-aminopyridine and tetraethylammonium ) , at concentrations without marked effects on K ( ir ) , failed to affect neurite extension .
	manualset3
97227	4	400150	5	NULL	NULL	0	NULL	K ( ir )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , other K + channel inhibitors ( 4-aminopyridine and tetraethylammonium ) , at concentrations without marked effects on K ( ir ) , failed to affect neurite extension .
	manualset3
97228	5	400150	5	NULL	NULL	0	NULL	affect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , other K + channel inhibitors ( 4-aminopyridine and tetraethylammonium ) , at concentrations without marked effects on K ( ir ) , failed to affect neurite extension .
	manualset3
97229	6	400150	5	NULL	NULL	0	NULL	neurite extension	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , other K + channel inhibitors ( 4-aminopyridine and tetraethylammonium ) , at concentrations without marked effects on K ( ir ) , failed to affect neurite extension .
	manualset3
97230	1	400151	5	NULL	NULL	0	NULL	celomic derivatives	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , other celomic derivatives , such as endometrium and endocervix , were negative for GHS-R1a immunoreactivity .
	manualset3
97231	2	400151	5	NULL	NULL	NULL	NULL	endometrium	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , other celomic derivatives , such as endometrium and endocervix , were negative for GHS-R1a immunoreactivity .
	manualset3
97232	3	400151	5	NULL	NULL	0	NULL	endocervix	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , other celomic derivatives , such as endometrium and endocervix , were negative for GHS-R1a immunoreactivity .
	manualset3
97233	4	400151	5	NULL	NULL	0	NULL	GHS-R1a immunoreactivity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , other celomic derivatives , such as endometrium and endocervix , were negative for GHS-R1a immunoreactivity .
	manualset3
97234	1	400152	5	NULL	NULL	0	NULL	ribavirin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , ribavirin at physiological doses had no effect on DC maturation but markedly suppressed the production of TNF-alpha , IL-10 , and IL-12 ( p70 ) .
	manualset3
97235	2	400152	5	NULL	NULL	0	NULL	physiological doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , ribavirin at physiological doses had no effect on DC maturation but markedly suppressed the production of TNF-alpha , IL-10 , and IL-12 ( p70 ) .
	manualset3
97236	3	400152	5	NULL	NULL	0	NULL	effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , ribavirin at physiological doses had no effect on DC maturation but markedly suppressed the production of TNF-alpha , IL-10 , and IL-12 ( p70 ) .
	manualset3
97237	4	400152	5	NULL	NULL	0	NULL	DC maturation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , ribavirin at physiological doses had no effect on DC maturation but markedly suppressed the production of TNF-alpha , IL-10 , and IL-12 ( p70 ) .
	manualset3
97238	5	400152	5	NULL	NULL	0	NULL	production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , ribavirin at physiological doses had no effect on DC maturation but markedly suppressed the production of TNF-alpha , IL-10 , and IL-12 ( p70 ) .
	manualset3
97239	6	400152	5	NULL	NULL	0	NULL	TNF-alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , ribavirin at physiological doses had no effect on DC maturation but markedly suppressed the production of TNF-alpha , IL-10 , and IL-12 ( p70 ) .
	manualset3
97240	7	400152	5	NULL	NULL	0	NULL	IL-10	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , ribavirin at physiological doses had no effect on DC maturation but markedly suppressed the production of TNF-alpha , IL-10 , and IL-12 ( p70 ) .
	manualset3
97241	8	400152	5	NULL	NULL	0	NULL	IL-12 ( p70 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , ribavirin at physiological doses had no effect on DC maturation but markedly suppressed the production of TNF-alpha , IL-10 , and IL-12 ( p70 ) .
	manualset3
97242	1	400153	5	NULL	NULL	0	NULL	40.10.09 antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the 40.10.09 antibody inhibited the activity of the two normal human lymphoblast enzymes .
	manualset3
97243	2	400153	5	NULL	NULL	0	NULL	activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the 40.10.09 antibody inhibited the activity of the two normal human lymphoblast enzymes .
	manualset3
97244	3	400153	5	NULL	NULL	0	NULL	normal human lymphoblast enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the 40.10.09 antibody inhibited the activity of the two normal human lymphoblast enzymes .
	manualset3
97245	1	400154	5	NULL	NULL	0	NULL	C19-cyc	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the C19-cyc and the 10-hydroxy acid ( C18 : 0 -10 OH ) species showed a noticeable decrease .
	manualset3
97246	2	400154	5	NULL	NULL	0	NULL	10-hydroxy acid ( C18 : 0 -10 OH ) species	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the C19-cyc and the 10-hydroxy acid ( C18 : 0 -10 OH ) species showed a noticeable decrease .
	manualset3
97247	1	400155	5	NULL	NULL	0	NULL	QA levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the QA levels in plasma , liver , spleen , and kidney were similar after a single 2 mg/kg i.v. dose and & lt ; 2 times greater after 10 mg/kg oral doses in MDR1-KO mice compared with WT mice .
	manualset3
97248	2	400155	5	NULL	NULL	0	NULL	plasma	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the QA levels in plasma , liver , spleen , and kidney were similar after a single 2 mg/kg i.v. dose and & lt ; 2 times greater after 10 mg/kg oral doses in MDR1-KO mice compared with WT mice .
	manualset3
97249	3	400155	5	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the QA levels in plasma , liver , spleen , and kidney were similar after a single 2 mg/kg i.v. dose and & lt ; 2 times greater after 10 mg/kg oral doses in MDR1-KO mice compared with WT mice .
	manualset3
97250	4	400155	5	NULL	NULL	0	NULL	spleen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the QA levels in plasma , liver , spleen , and kidney were similar after a single 2 mg/kg i.v. dose and & lt ; 2 times greater after 10 mg/kg oral doses in MDR1-KO mice compared with WT mice .
	manualset3
97251	5	400155	5	NULL	NULL	0	NULL	kidney	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the QA levels in plasma , liver , spleen , and kidney were similar after a single 2 mg/kg i.v. dose and & lt ; 2 times greater after 10 mg/kg oral doses in MDR1-KO mice compared with WT mice .
	manualset3
97252	6	400155	5	NULL	NULL	NULL	NULL	single 2 mg/kg	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , the QA levels in plasma , liver , spleen , and kidney were similar after a single 2 mg/kg i.v. dose and & lt ; 2 times greater after 10 mg/kg oral doses in MDR1-KO mice compared with WT mice .
	manualset3
97253	8	400155	5	NULL	NULL	NULL	NULL	2 times greater	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , the QA levels in plasma , liver , spleen , and kidney were similar after a single 2 mg/kg i.v. dose and & lt ; 2 times greater after 10 mg/kg oral doses in MDR1-KO mice compared with WT mice .
	manualset3
97254	7	400155	5	NULL	NULL	0	NULL	i.v. dose and & lt	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the QA levels in plasma , liver , spleen , and kidney were similar after a single 2 mg/kg i.v. dose and & lt ; 2 times greater after 10 mg/kg oral doses in MDR1-KO mice compared with WT mice .
	manualset3
97255	9	400155	5	NULL	NULL	0	NULL	10 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the QA levels in plasma , liver , spleen , and kidney were similar after a single 2 mg/kg i.v. dose and & lt ; 2 times greater after 10 mg/kg oral doses in MDR1-KO mice compared with WT mice .
	manualset3
97256	10	400155	5	NULL	NULL	0	NULL	oral doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the QA levels in plasma , liver , spleen , and kidney were similar after a single 2 mg/kg i.v. dose and & lt ; 2 times greater after 10 mg/kg oral doses in MDR1-KO mice compared with WT mice .
	manualset3
97257	11	400155	5	NULL	NULL	0	NULL	MDR1-KO mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the QA levels in plasma , liver , spleen , and kidney were similar after a single 2 mg/kg i.v. dose and & lt ; 2 times greater after 10 mg/kg oral doses in MDR1-KO mice compared with WT mice .
	manualset3
97258	12	400155	5	NULL	NULL	0	NULL	WT mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the QA levels in plasma , liver , spleen , and kidney were similar after a single 2 mg/kg i.v. dose and & lt ; 2 times greater after 10 mg/kg oral doses in MDR1-KO mice compared with WT mice .
	manualset3
97259	1	400156	5	NULL	NULL	0	NULL	W171A variant 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the W171A variant was unable to oxidize VA , confirming the apparent essentiality of Trp171 in VA oxidation by LiP .
	manualset3
97260	2	400156	5	NULL	NULL	0	NULL	oxidize	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the W171A variant was unable to oxidize VA , confirming the apparent essentiality of Trp171 in VA oxidation by LiP .
	manualset3
97261	3	400156	5	NULL	NULL	0	NULL	VA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the W171A variant was unable to oxidize VA , confirming the apparent essentiality of Trp171 in VA oxidation by LiP .
	manualset3
97262	4	400156	5	NULL	NULL	0	NULL	apparent essentiality	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the W171A variant was unable to oxidize VA , confirming the apparent essentiality of Trp171 in VA oxidation by LiP .
	manualset3
97263	5	400156	5	NULL	NULL	0	NULL	Trp171	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the W171A variant was unable to oxidize VA , confirming the apparent essentiality of Trp171 in VA oxidation by LiP .
	manualset3
97264	6	400156	5	NULL	NULL	0	NULL	VA oxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the W171A variant was unable to oxidize VA , confirming the apparent essentiality of Trp171 in VA oxidation by LiP .
	manualset3
97265	7	400156	5	NULL	NULL	0	NULL	LiP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the W171A variant was unable to oxidize VA , confirming the apparent essentiality of Trp171 in VA oxidation by LiP .
	manualset3
97266	7	400156	5	NULL	NULL	0	NULL	LiP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the W171A variant was unable to oxidize VA , confirming the apparent essentiality of Trp171 in VA oxidation by LiP .
	manualset3
97267	1	400157	5	NULL	NULL	NULL	NULL	absolute tetanic tension	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , the absolute tetanic tension of the EDL was reduced ( P & lt ; 0.01 ) in mdx mice compared to C57BL/10 mice , and both relative twitch and tetanic tensions were also lower ( P & lt ; 0.001 ) in mdx mice .
	manualset3
97268	2	400157	5	NULL	NULL	0	NULL	EDL	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the absolute tetanic tension of the EDL was reduced ( P & lt ; 0.01 ) in mdx mice compared to C57BL/10 mice , and both relative twitch and tetanic tensions were also lower ( P & lt ; 0.001 ) in mdx mice .
	manualset3
97269	3	400157	5	NULL	NULL	0	NULL	P & lt ; 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the absolute tetanic tension of the EDL was reduced ( P & lt ; 0.01 ) in mdx mice compared to C57BL/10 mice , and both relative twitch and tetanic tensions were also lower ( P & lt ; 0.001 ) in mdx mice .
	manualset3
97270	4	400157	5	NULL	NULL	0	NULL	mdx mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the absolute tetanic tension of the EDL was reduced ( P & lt ; 0.01 ) in mdx mice compared to C57BL/10 mice , and both relative twitch and tetanic tensions were also lower ( P & lt ; 0.001 ) in mdx mice .
	manualset3
97271	5	400157	5	NULL	NULL	0	NULL	C57BL/10 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the absolute tetanic tension of the EDL was reduced ( P & lt ; 0.01 ) in mdx mice compared to C57BL/10 mice , and both relative twitch and tetanic tensions were also lower ( P & lt ; 0.001 ) in mdx mice .
	manualset3
97272	6	400157	5	NULL	NULL	0	NULL	relative twitch	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the absolute tetanic tension of the EDL was reduced ( P & lt ; 0.01 ) in mdx mice compared to C57BL/10 mice , and both relative twitch and tetanic tensions were also lower ( P & lt ; 0.001 ) in mdx mice .
	manualset3
97273	7	400157	5	NULL	NULL	0	NULL	tetanic tensions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the absolute tetanic tension of the EDL was reduced ( P & lt ; 0.01 ) in mdx mice compared to C57BL/10 mice , and both relative twitch and tetanic tensions were also lower ( P & lt ; 0.001 ) in mdx mice .
	manualset3
97274	8	400157	5	NULL	NULL	0	NULL	 P & lt ; 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the absolute tetanic tension of the EDL was reduced ( P & lt ; 0.01 ) in mdx mice compared to C57BL/10 mice , and both relative twitch and tetanic tensions were also lower ( P & lt ; 0.001 ) in mdx mice .
	manualset3
97275	9	400157	5	NULL	NULL	0	NULL	mdx mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the absolute tetanic tension of the EDL was reduced ( P & lt ; 0.01 ) in mdx mice compared to C57BL/10 mice , and both relative twitch and tetanic tensions were also lower ( P & lt ; 0.001 ) in mdx mice .
	manualset3
97276	1	400158	5	NULL	NULL	0	NULL	actions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the actions of HGF on sensory neurons are mediated by Met effectors distinct from Grb2 .
	manualset3
97277	2	400158	5	NULL	NULL	0	NULL	HGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the actions of HGF on sensory neurons are mediated by Met effectors distinct from Grb2 .
	manualset3
97278	3	400158	5	NULL	NULL	0	NULL	sensory neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the actions of HGF on sensory neurons are mediated by Met effectors distinct from Grb2 .
	manualset3
97279	4	400158	5	NULL	NULL	NULL	NULL	Met effectors	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , the actions of HGF on sensory neurons are mediated by Met effectors distinct from Grb2 .
	manualset3
97280	5	400158	5	NULL	NULL	0	NULL	Grb2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the actions of HGF on sensory neurons are mediated by Met effectors distinct from Grb2 .
	manualset3
97281	1	400159	5	NULL	NULL	0	NULL	risk 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( What is the risk of developing hepatocarcinoma in primary biliary cirrhosis ? ) .
	manualset3
97282	2	400159	5	NULL	NULL	0	NULL	hepatocarcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( What is the risk of developing hepatocarcinoma in primary biliary cirrhosis ? ) .
	manualset3
97283	3	400159	5	NULL	NULL	0	NULL	primary biliary cirrhosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( What is the risk of developing hepatocarcinoma in primary biliary cirrhosis ? ) .
	manualset3
97284	1	400160	5	NULL	NULL	0	NULL	activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the activity of creatine kinase remained depressed throughout the same period .
	manualset3
97285	2	400160	5	NULL	NULL	0	NULL	creatine kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the activity of creatine kinase remained depressed throughout the same period .
	manualset3
97286	3	400160	5	NULL	NULL	0	NULL	period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the activity of creatine kinase remained depressed throughout the same period .
	manualset3
97287	1	400161	5	NULL	NULL	NULL	NULL	antioxidants , butylated hydroxytoluene	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , the antioxidants , butylated hydroxytoluene and Trolox C , and the iron-chelating agent , deferoxamine , suppressed allyl alcohol-induced MDA production without affecting the depletion of cellular thiols or the loss of viability .
	manualset3
97288	2	400161	5	NULL	NULL	NULL	NULL	antioxidants, Trolox C	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , the antioxidants , butylated hydroxytoluene and Trolox C , and the iron-chelating agent , deferoxamine , suppressed allyl alcohol-induced MDA production without affecting the depletion of cellular thiols or the loss of viability .
	manualset3
97289	3	400161	5	NULL	NULL	NULL	NULL	iron-chelating agent , deferoxamine	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , the antioxidants , butylated hydroxytoluene and Trolox C , and the iron-chelating agent , deferoxamine , suppressed allyl alcohol-induced MDA production without affecting the depletion of cellular thiols or the loss of viability .
	manualset3
97290	4	400161	5	NULL	NULL	0	NULL	allyl alcohol-induced MDA production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the antioxidants , butylated hydroxytoluene and Trolox C , and the iron-chelating agent , deferoxamine , suppressed allyl alcohol-induced MDA production without affecting the depletion of cellular thiols or the loss of viability .
	manualset3
97291	5	400161	5	NULL	NULL	0	NULL	depletion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the antioxidants , butylated hydroxytoluene and Trolox C , and the iron-chelating agent , deferoxamine , suppressed allyl alcohol-induced MDA production without affecting the depletion of cellular thiols or the loss of viability .
	manualset3
97292	6	400161	5	NULL	NULL	0	NULL	cellular thiols	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the antioxidants , butylated hydroxytoluene and Trolox C , and the iron-chelating agent , deferoxamine , suppressed allyl alcohol-induced MDA production without affecting the depletion of cellular thiols or the loss of viability .
	manualset3
97293	7	400161	5	NULL	NULL	0	NULL	viability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the antioxidants , butylated hydroxytoluene and Trolox C , and the iron-chelating agent , deferoxamine , suppressed allyl alcohol-induced MDA production without affecting the depletion of cellular thiols or the loss of viability .
	manualset3
97294	1	400162	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the effects of asbestos were minimal in 0 SAE cells .
	manualset3
97295	2	400162	5	NULL	NULL	0	NULL	asbestos	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the effects of asbestos were minimal in 0 SAE cells .
	manualset3
97296	3	400162	5	NULL	NULL	0	NULL	0 SAE cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the effects of asbestos were minimal in 0 SAE cells .
	manualset3
97297	1	400163	5	NULL	NULL	0	NULL	levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the levels of phospholipase A2 , enkephalin , PSD-95 , synaptophysin , or glutamate NMDA receptor subunit type 2B were either unaltered in AD mice or unaffected by treatment .
	manualset3
97298	2	400163	5	NULL	NULL	0	NULL	phospholipase A2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the levels of phospholipase A2 , enkephalin , PSD-95 , synaptophysin , or glutamate NMDA receptor subunit type 2B were either unaltered in AD mice or unaffected by treatment .
	manualset3
97299	3	400163	5	NULL	NULL	0	NULL	enkephalin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the levels of phospholipase A2 , enkephalin , PSD-95 , synaptophysin , or glutamate NMDA receptor subunit type 2B were either unaltered in AD mice or unaffected by treatment .
	manualset3
97300	4	400163	5	NULL	NULL	0	NULL	PSD-95	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the levels of phospholipase A2 , enkephalin , PSD-95 , synaptophysin , or glutamate NMDA receptor subunit type 2B were either unaltered in AD mice or unaffected by treatment .
	manualset3
97301	5	400163	5	NULL	NULL	0	NULL	synaptophysin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the levels of phospholipase A2 , enkephalin , PSD-95 , synaptophysin , or glutamate NMDA receptor subunit type 2B were either unaltered in AD mice or unaffected by treatment .
	manualset3
97302	6	400163	5	NULL	NULL	0	NULL	glutamate NMDA receptor subunit type 2B 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the levels of phospholipase A2 , enkephalin , PSD-95 , synaptophysin , or glutamate NMDA receptor subunit type 2B were either unaltered in AD mice or unaffected by treatment .
	manualset3
97303	7	400163	5	NULL	NULL	0	NULL	AD mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the levels of phospholipase A2 , enkephalin , PSD-95 , synaptophysin , or glutamate NMDA receptor subunit type 2B were either unaltered in AD mice or unaffected by treatment .
	manualset3
97304	8	400163	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the levels of phospholipase A2 , enkephalin , PSD-95 , synaptophysin , or glutamate NMDA receptor subunit type 2B were either unaltered in AD mice or unaffected by treatment .
	manualset3
97305	1	400164	5	NULL	NULL	NULL	NULL	mechanism	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , the mechanism of eigenmode synchronization critically depends on the geometrical and biomechanical properties of the vocal folds ( at least 2-degrees-of-freedom are required ) , and has little requirement on the glottal aerodynamics other than flow separation .
	manualset3
97306	2	400164	5	NULL	NULL	NULL	NULL	eigenmode synchronization	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , the mechanism of eigenmode synchronization critically depends on the geometrical and biomechanical properties of the vocal folds ( at least 2-degrees-of-freedom are required ) , and has little requirement on the glottal aerodynamics other than flow separation .
	manualset3
97307	3	400164	5	NULL	NULL	0	NULL	geometrical and biomechanical properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the mechanism of eigenmode synchronization critically depends on the geometrical and biomechanical properties of the vocal folds ( at least 2-degrees-of-freedom are required ) , and has little requirement on the glottal aerodynamics other than flow separation .
	manualset3
97308	4	400164	5	NULL	NULL	0	NULL	vocal folds	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the mechanism of eigenmode synchronization critically depends on the geometrical and biomechanical properties of the vocal folds ( at least 2-degrees-of-freedom are required ) , and has little requirement on the glottal aerodynamics other than flow separation .
	manualset3
97309	5	400164	5	NULL	NULL	0	NULL	2-degrees-of-freedom	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the mechanism of eigenmode synchronization critically depends on the geometrical and biomechanical properties of the vocal folds ( at least 2-degrees-of-freedom are required ) , and has little requirement on the glottal aerodynamics other than flow separation .
	manualset3
97310	6	400164	5	NULL	NULL	0	NULL	glottal aerodynamics	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the mechanism of eigenmode synchronization critically depends on the geometrical and biomechanical properties of the vocal folds ( at least 2-degrees-of-freedom are required ) , and has little requirement on the glottal aerodynamics other than flow separation .
	manualset3
97311	7	400164	5	NULL	NULL	0	NULL	flow separation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the mechanism of eigenmode synchronization critically depends on the geometrical and biomechanical properties of the vocal folds ( at least 2-degrees-of-freedom are required ) , and has little requirement on the glottal aerodynamics other than flow separation .
	manualset3
97312	1	400165	5	NULL	NULL	0	NULL	mitochondrial surface area	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the mitochondrial surface area of the right atrium showed a mean increase of 65.8 % , from 0.231 + / - 0.038 micron 2 in the preischemic stage to 0.383 + / - 0.057 micron 2 in the ischemic stage ( p less than 0.001 ) .
	manualset3
97313	2	400165	5	NULL	NULL	0	NULL	right atrium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the mitochondrial surface area of the right atrium showed a mean increase of 65.8 % , from 0.231 + / - 0.038 micron 2 in the preischemic stage to 0.383 + / - 0.057 micron 2 in the ischemic stage ( p less than 0.001 ) .
	manualset3
97314	3	400165	5	NULL	NULL	0	NULL	65.8 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the mitochondrial surface area of the right atrium showed a mean increase of 65.8 % , from 0.231 + / - 0.038 micron 2 in the preischemic stage to 0.383 + / - 0.057 micron 2 in the ischemic stage ( p less than 0.001 ) .
	manualset3
97315	4	400165	5	NULL	NULL	0	NULL	0.231 + / - 0.038 micron 2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the mitochondrial surface area of the right atrium showed a mean increase of 65.8 % , from 0.231 + / - 0.038 micron 2 in the preischemic stage to 0.383 + / - 0.057 micron 2 in the ischemic stage ( p less than 0.001 ) .
	manualset3
97316	5	400165	5	NULL	NULL	0	NULL	preischemic stage	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the mitochondrial surface area of the right atrium showed a mean increase of 65.8 % , from 0.231 + / - 0.038 micron 2 in the preischemic stage to 0.383 + / - 0.057 micron 2 in the ischemic stage ( p less than 0.001 ) .
	manualset3
97317	6	400165	5	NULL	NULL	0	NULL	0.383 + / - 0.057 micron 2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the mitochondrial surface area of the right atrium showed a mean increase of 65.8 % , from 0.231 + / - 0.038 micron 2 in the preischemic stage to 0.383 + / - 0.057 micron 2 in the ischemic stage ( p less than 0.001 ) .
	manualset3
97318	7	400165	5	NULL	NULL	0	NULL	ischemic stage	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the mitochondrial surface area of the right atrium showed a mean increase of 65.8 % , from 0.231 + / - 0.038 micron 2 in the preischemic stage to 0.383 + / - 0.057 micron 2 in the ischemic stage ( p less than 0.001 ) .
	manualset3
97319	8	400165	5	NULL	NULL	0	NULL	 p less than 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the mitochondrial surface area of the right atrium showed a mean increase of 65.8 % , from 0.231 + / - 0.038 micron 2 in the preischemic stage to 0.383 + / - 0.057 micron 2 in the ischemic stage ( p less than 0.001 ) .
	manualset3
97320	1	400166	5	NULL	NULL	0	NULL	nonhabituated aroused rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the nonhabituated aroused rats were impaired when consolidation was examined , but their memory was intact following reactivation of the memory trace .
	manualset3
97321	2	400166	5	NULL	NULL	0	NULL	consolidation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the nonhabituated aroused rats were impaired when consolidation was examined , but their memory was intact following reactivation of the memory trace .
	manualset3
97322	3	400166	5	NULL	NULL	0	NULL	memory	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the nonhabituated aroused rats were impaired when consolidation was examined , but their memory was intact following reactivation of the memory trace .
	manualset3
97323	4	400166	5	NULL	NULL	0	NULL	reactivation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the nonhabituated aroused rats were impaired when consolidation was examined , but their memory was intact following reactivation of the memory trace .
	manualset3
97324	5	400166	5	NULL	NULL	0	NULL	memory trace	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the nonhabituated aroused rats were impaired when consolidation was examined , but their memory was intact following reactivation of the memory trace .
	manualset3
97325	1	400167	5	NULL	NULL	NULL	NULL	ob/ob mouse islets	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , the ob/ob mouse islets at 5.5 mM glucose dephosphorylated 18 % of the glucose phosphorylated and 30 % at 16.7 mM .
	manualset3
97326	2	400167	5	NULL	NULL	0	NULL	5.5 mM glucose	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the ob/ob mouse islets at 5.5 mM glucose dephosphorylated 18 % of the glucose phosphorylated and 30 % at 16.7 mM .
	manualset3
97327	3	400167	5	NULL	NULL	0	NULL	18 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the ob/ob mouse islets at 5.5 mM glucose dephosphorylated 18 % of the glucose phosphorylated and 30 % at 16.7 mM .
	manualset3
97328	4	400167	5	NULL	NULL	0	NULL	glucose	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the ob/ob mouse islets at 5.5 mM glucose dephosphorylated 18 % of the glucose phosphorylated and 30 % at 16.7 mM .
	manualset3
97329	5	400167	5	NULL	NULL	0	NULL	30 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the ob/ob mouse islets at 5.5 mM glucose dephosphorylated 18 % of the glucose phosphorylated and 30 % at 16.7 mM .
	manualset3
97330	6	400167	5	NULL	NULL	0	NULL	16.7 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the ob/ob mouse islets at 5.5 mM glucose dephosphorylated 18 % of the glucose phosphorylated and 30 % at 16.7 mM .
	manualset3
97331	1	400168	5	NULL	NULL	0	NULL	incretin hormone , glucagon-like peptide-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the other major incretin hormone , glucagon-like peptide-1 , exhibited no significant effects on LPL activity or PKB , LKB1 , or AMPK phosphorylation .
	manualset3
97332	2	400168	5	NULL	NULL	0	NULL	significant effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the other major incretin hormone , glucagon-like peptide-1 , exhibited no significant effects on LPL activity or PKB , LKB1 , or AMPK phosphorylation .
	manualset3
97333	3	400168	5	NULL	NULL	0	NULL	LPL activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the other major incretin hormone , glucagon-like peptide-1 , exhibited no significant effects on LPL activity or PKB , LKB1 , or AMPK phosphorylation .
	manualset3
97334	4	400168	5	NULL	NULL	0	NULL	PKB phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the other major incretin hormone , glucagon-like peptide-1 , exhibited no significant effects on LPL activity or PKB , LKB1 , or AMPK phosphorylation .
	manualset3
97335	5	400168	5	NULL	NULL	0	NULL	LKB1 phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the other major incretin hormone , glucagon-like peptide-1 , exhibited no significant effects on LPL activity or PKB , LKB1 , or AMPK phosphorylation .
	manualset3
97336	6	400168	5	NULL	NULL	0	NULL	AMPK phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the other major incretin hormone , glucagon-like peptide-1 , exhibited no significant effects on LPL activity or PKB , LKB1 , or AMPK phosphorylation .
	manualset3
97337	1	400169	5	NULL	NULL	0	NULL	outcome	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the outcome of emergency liver transplantation was dismal in three cases of exertional heatstroke in the literature .
	manualset3
97406	2	400169	5	NULL	NULL	0	NULL	emergency liver transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the outcome of emergency liver transplantation was dismal in three cases of exertional heatstroke in the literature .
	manualset3
97407	3	400169	5	NULL	NULL	0	NULL	three cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the outcome of emergency liver transplantation was dismal in three cases of exertional heatstroke in the literature .
	manualset3
97408	4	400169	5	NULL	NULL	0	NULL	exertional heatstroke	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the outcome of emergency liver transplantation was dismal in three cases of exertional heatstroke in the literature .
	manualset3
97409	5	400169	5	NULL	NULL	0	NULL	literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the outcome of emergency liver transplantation was dismal in three cases of exertional heatstroke in the literature .
	manualset3
97562	1	400170	5	NULL	NULL	0	NULL	persistence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the persistence of false positives with the two methods and the impossibility of distinguishing between inflammatory lymph nodes and neoplastic lymph nodes means that thoracotomy can never be contraindicated on the basis of the results of imaging alone .
	manualset3
97563	2	400170	5	NULL	NULL	0	NULL	false positives	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the persistence of false positives with the two methods and the impossibility of distinguishing between inflammatory lymph nodes and neoplastic lymph nodes means that thoracotomy can never be contraindicated on the basis of the results of imaging alone .
	manualset3
97564	3	400170	5	NULL	NULL	0	NULL	two methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the persistence of false positives with the two methods and the impossibility of distinguishing between inflammatory lymph nodes and neoplastic lymph nodes means that thoracotomy can never be contraindicated on the basis of the results of imaging alone .
	manualset3
97565	4	400170	5	NULL	NULL	0	NULL	inflammatory lymph nodes 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the persistence of false positives with the two methods and the impossibility of distinguishing between inflammatory lymph nodes and neoplastic lymph nodes means that thoracotomy can never be contraindicated on the basis of the results of imaging alone .
	manualset3
97566	5	400170	5	NULL	NULL	0	NULL	neoplastic lymph nodes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the persistence of false positives with the two methods and the impossibility of distinguishing between inflammatory lymph nodes and neoplastic lymph nodes means that thoracotomy can never be contraindicated on the basis of the results of imaging alone .
	manualset3
97567	6	400170	5	NULL	NULL	0	NULL	thoracotomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the persistence of false positives with the two methods and the impossibility of distinguishing between inflammatory lymph nodes and neoplastic lymph nodes means that thoracotomy can never be contraindicated on the basis of the results of imaging alone .
	manualset3
97568	7	400170	5	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the persistence of false positives with the two methods and the impossibility of distinguishing between inflammatory lymph nodes and neoplastic lymph nodes means that thoracotomy can never be contraindicated on the basis of the results of imaging alone .
	manualset3
97569	1	400171	5	NULL	NULL	NULL	NULL	amount	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , the same amount of purified SHBG added to MCF-7 cells expressing wild type SHBG partially inhibited the estradiol-induced cell proliferation .
	manualset3
97570	2	400171	5	NULL	NULL	0	NULL	purified SHBG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the same amount of purified SHBG added to MCF-7 cells expressing wild type SHBG partially inhibited the estradiol-induced cell proliferation .
	manualset3
97571	3	400171	5	NULL	NULL	0	NULL	MCF-7 cells expressing wild type SHBG 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the same amount of purified SHBG added to MCF-7 cells expressing wild type SHBG partially inhibited the estradiol-induced cell proliferation .
	manualset3
97572	4	400171	5	NULL	NULL	NULL	NULL	estradiol-induced cell proliferation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , the same amount of purified SHBG added to MCF-7 cells expressing wild type SHBG partially inhibited the estradiol-induced cell proliferation .
	manualset3
97573	1	400172	5	NULL	NULL	0	NULL	IgG autoantibody fingerprints	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the sharing of IgG autoantibody fingerprints by monozygotic twins suggests that lupus IgG autoantibodies can arise in predisposed individuals in genetically determined patterns .
	manualset3
97574	2	400172	5	NULL	NULL	0	NULL	monozygotic twins	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the sharing of IgG autoantibody fingerprints by monozygotic twins suggests that lupus IgG autoantibodies can arise in predisposed individuals in genetically determined patterns .
	manualset3
97575	3	400172	5	NULL	NULL	NULL	NULL	lupus IgG autoantibodies	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , the sharing of IgG autoantibody fingerprints by monozygotic twins suggests that lupus IgG autoantibodies can arise in predisposed individuals in genetically determined patterns .
	manualset3
97576	4	400172	5	NULL	NULL	0	NULL	predisposed individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the sharing of IgG autoantibody fingerprints by monozygotic twins suggests that lupus IgG autoantibodies can arise in predisposed individuals in genetically determined patterns .
	manualset3
97577	5	400172	5	NULL	NULL	0	NULL	genetically determined patterns	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the sharing of IgG autoantibody fingerprints by monozygotic twins suggests that lupus IgG autoantibodies can arise in predisposed individuals in genetically determined patterns .
	manualset3
98195	1	400173	5	NULL	NULL	0	NULL	solvated species ( Fe ( L ) ( DBC ) ( Sol ) ) ( + )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the solvated species ( Fe ( L ) ( DBC ) ( Sol ) ) ( + ) derived from 5-8 cleave H ( 2 ) DBC to provide both extradiol and intradiol products ( E/I , 0.6 : 1 -2.3 : 1 ) due to the involvement of the ether oxygen donor of the methoxyethyl/tetrahydrofuryl arm in the coordination to iron ( III ) upon removal of a chloride ion .
	manualset3
98196	2	400173	5	NULL	NULL	0	NULL	5-8 cleave H ( 2 ) DBC	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the solvated species ( Fe ( L ) ( DBC ) ( Sol ) ) ( + ) derived from 5-8 cleave H ( 2 ) DBC to provide both extradiol and intradiol products ( E/I , 0.6 : 1 -2.3 : 1 ) due to the involvement of the ether oxygen donor of the methoxyethyl/tetrahydrofuryl arm in the coordination to iron ( III ) upon removal of a chloride ion .
	manualset3
98197	3	400173	5	NULL	NULL	NULL	NULL	extradiol products	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , the solvated species ( Fe ( L ) ( DBC ) ( Sol ) ) ( + ) derived from 5-8 cleave H ( 2 ) DBC to provide both extradiol and intradiol products ( E/I , 0.6 : 1 -2.3 : 1 ) due to the involvement of the ether oxygen donor of the methoxyethyl/tetrahydrofuryl arm in the coordination to iron ( III ) upon removal of a chloride ion .
	manualset3
98198	4	400173	5	NULL	NULL	0	NULL	intradiol products	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the solvated species ( Fe ( L ) ( DBC ) ( Sol ) ) ( + ) derived from 5-8 cleave H ( 2 ) DBC to provide both extradiol and intradiol products ( E/I , 0.6 : 1 -2.3 : 1 ) due to the involvement of the ether oxygen donor of the methoxyethyl/tetrahydrofuryl arm in the coordination to iron ( III ) upon removal of a chloride ion .
	manualset3
98199	5	400173	5	NULL	NULL	0	NULL	E/I , 0.6 : 1 -2.3 : 1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the solvated species ( Fe ( L ) ( DBC ) ( Sol ) ) ( + ) derived from 5-8 cleave H ( 2 ) DBC to provide both extradiol and intradiol products ( E/I , 0.6 : 1 -2.3 : 1 ) due to the involvement of the ether oxygen donor of the methoxyethyl/tetrahydrofuryl arm in the coordination to iron ( III ) upon removal of a chloride ion .
	manualset3
98200	6	400173	5	NULL	NULL	0	NULL	involvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the solvated species ( Fe ( L ) ( DBC ) ( Sol ) ) ( + ) derived from 5-8 cleave H ( 2 ) DBC to provide both extradiol and intradiol products ( E/I , 0.6 : 1 -2.3 : 1 ) due to the involvement of the ether oxygen donor of the methoxyethyl/tetrahydrofuryl arm in the coordination to iron ( III ) upon removal of a chloride ion .
	manualset3
98201	7	400173	5	NULL	NULL	0	NULL	oxygen donor	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the solvated species ( Fe ( L ) ( DBC ) ( Sol ) ) ( + ) derived from 5-8 cleave H ( 2 ) DBC to provide both extradiol and intradiol products ( E/I , 0.6 : 1 -2.3 : 1 ) due to the involvement of the ether oxygen donor of the methoxyethyl/tetrahydrofuryl arm in the coordination to iron ( III ) upon removal of a chloride ion .
	manualset3
98202	8	400173	5	NULL	NULL	0	NULL	methoxyethyl/tetrahydrofuryl arm	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the solvated species ( Fe ( L ) ( DBC ) ( Sol ) ) ( + ) derived from 5-8 cleave H ( 2 ) DBC to provide both extradiol and intradiol products ( E/I , 0.6 : 1 -2.3 : 1 ) due to the involvement of the ether oxygen donor of the methoxyethyl/tetrahydrofuryl arm in the coordination to iron ( III ) upon removal of a chloride ion .
	manualset3
98203	9	400173	5	NULL	NULL	0	NULL	iron(III)	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the solvated species ( Fe ( L ) ( DBC ) ( Sol ) ) ( + ) derived from 5-8 cleave H ( 2 ) DBC to provide both extradiol and intradiol products ( E/I , 0.6 : 1 -2.3 : 1 ) due to the involvement of the ether oxygen donor of the methoxyethyl/tetrahydrofuryl arm in the coordination to iron ( III ) upon removal of a chloride ion .
	manualset3
98204	10	400173	5	NULL	NULL	0	NULL	removal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the solvated species ( Fe ( L ) ( DBC ) ( Sol ) ) ( + ) derived from 5-8 cleave H ( 2 ) DBC to provide both extradiol and intradiol products ( E/I , 0.6 : 1 -2.3 : 1 ) due to the involvement of the ether oxygen donor of the methoxyethyl/tetrahydrofuryl arm in the coordination to iron ( III ) upon removal of a chloride ion .
	manualset3
98205	11	400173	5	NULL	NULL	0	NULL	chloride ion	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the solvated species ( Fe ( L ) ( DBC ) ( Sol ) ) ( + ) derived from 5-8 cleave H ( 2 ) DBC to provide both extradiol and intradiol products ( E/I , 0.6 : 1 -2.3 : 1 ) due to the involvement of the ether oxygen donor of the methoxyethyl/tetrahydrofuryl arm in the coordination to iron ( III ) upon removal of a chloride ion .
	manualset3
98206	1	400174	5	NULL	NULL	NULL	NULL	tetramer-dimer dissociation constants	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , the tetramer-dimer dissociation constants of deoxyhemoglobins A and Kansas appear to be identical .
	manualset3
98207	2	400174	5	NULL	NULL	0	NULL	deoxyhemoglobins A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the tetramer-dimer dissociation constants of deoxyhemoglobins A and Kansas appear to be identical .
	manualset3
98208	3	400174	5	NULL	NULL	0	NULL	deoxyhemoglobin Kansas	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the tetramer-dimer dissociation constants of deoxyhemoglobins A and Kansas appear to be identical .
	manualset3
98209	1	400175	5	NULL	NULL	0	NULL	urine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the urine of subjects infused with hCG has been shown to contain hCG itself , but nil beta-CTP fragments or as-hCG .
	manualset3
98210	2	400175	5	NULL	NULL	0	NULL	subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the urine of subjects infused with hCG has been shown to contain hCG itself , but nil beta-CTP fragments or as-hCG .
	manualset3
98211	3	400175	5	NULL	NULL	0	NULL	hCG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the urine of subjects infused with hCG has been shown to contain hCG itself , but nil beta-CTP fragments or as-hCG .
	manualset3
98212	4	400175	5	NULL	NULL	0	NULL	hCG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the urine of subjects infused with hCG has been shown to contain hCG itself , but nil beta-CTP fragments or as-hCG .
	manualset3
98213	5	400175	5	NULL	NULL	0	NULL	beta-CTP fragments	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the urine of subjects infused with hCG has been shown to contain hCG itself , but nil beta-CTP fragments or as-hCG .
	manualset3
98214	6	400175	5	NULL	NULL	0	NULL	as-hCG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the urine of subjects infused with hCG has been shown to contain hCG itself , but nil beta-CTP fragments or as-hCG .
	manualset3
98215	1	400176	5	NULL	NULL	0	NULL	significant interaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there was a significant interaction of training and hypoxia ( P & lt ; 0.05 ) on glucose metabolism , as follows : plasma insulin and glucose concentrations were significantly increased ; glucose metabolic clearance rate was decreased ; and the insulin to glucagon ratio was increased after training in the HYP group .
	manualset3
98216	2	400176	5	NULL	NULL	0	NULL	training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there was a significant interaction of training and hypoxia ( P & lt ; 0.05 ) on glucose metabolism , as follows : plasma insulin and glucose concentrations were significantly increased ; glucose metabolic clearance rate was decreased ; and the insulin to glucagon ratio was increased after training in the HYP group .
	manualset3
98217	3	400176	5	NULL	NULL	0	NULL	hypoxia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there was a significant interaction of training and hypoxia ( P & lt ; 0.05 ) on glucose metabolism , as follows : plasma insulin and glucose concentrations were significantly increased ; glucose metabolic clearance rate was decreased ; and the insulin to glucagon ratio was increased after training in the HYP group .
	manualset3
98218	4	400176	5	NULL	NULL	0	NULL	( P & lt ; 0.05 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there was a significant interaction of training and hypoxia ( P & lt ; 0.05 ) on glucose metabolism , as follows : plasma insulin and glucose concentrations were significantly increased ; glucose metabolic clearance rate was decreased ; and the insulin to glucagon ratio was increased after training in the HYP group .
	manualset3
98219	5	400176	5	NULL	NULL	0	NULL	glucose metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there was a significant interaction of training and hypoxia ( P & lt ; 0.05 ) on glucose metabolism , as follows : plasma insulin and glucose concentrations were significantly increased ; glucose metabolic clearance rate was decreased ; and the insulin to glucagon ratio was increased after training in the HYP group .
	manualset3
98220	6	400176	5	NULL	NULL	0	NULL	plasma insulin concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there was a significant interaction of training and hypoxia ( P & lt ; 0.05 ) on glucose metabolism , as follows : plasma insulin and glucose concentrations were significantly increased ; glucose metabolic clearance rate was decreased ; and the insulin to glucagon ratio was increased after training in the HYP group .
	manualset3
98221	7	400176	5	NULL	NULL	0	NULL	plasma glucose concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there was a significant interaction of training and hypoxia ( P & lt ; 0.05 ) on glucose metabolism , as follows : plasma insulin and glucose concentrations were significantly increased ; glucose metabolic clearance rate was decreased ; and the insulin to glucagon ratio was increased after training in the HYP group .
	manualset3
98222	8	400176	5	NULL	NULL	0	NULL	glucose metabolic clearance rate	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there was a significant interaction of training and hypoxia ( P & lt ; 0.05 ) on glucose metabolism , as follows : plasma insulin and glucose concentrations were significantly increased ; glucose metabolic clearance rate was decreased ; and the insulin to glucagon ratio was increased after training in the HYP group .
	manualset3
98223	9	400176	5	NULL	NULL	0	NULL	insulin to glucagon ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there was a significant interaction of training and hypoxia ( P & lt ; 0.05 ) on glucose metabolism , as follows : plasma insulin and glucose concentrations were significantly increased ; glucose metabolic clearance rate was decreased ; and the insulin to glucagon ratio was increased after training in the HYP group .
	manualset3
98224	10	400176	5	NULL	NULL	0	NULL	training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there was a significant interaction of training and hypoxia ( P & lt ; 0.05 ) on glucose metabolism , as follows : plasma insulin and glucose concentrations were significantly increased ; glucose metabolic clearance rate was decreased ; and the insulin to glucagon ratio was increased after training in the HYP group .
	manualset3
98225	11	400176	5	NULL	NULL	0	NULL	HYP group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there was a significant interaction of training and hypoxia ( P & lt ; 0.05 ) on glucose metabolism , as follows : plasma insulin and glucose concentrations were significantly increased ; glucose metabolic clearance rate was decreased ; and the insulin to glucagon ratio was increased after training in the HYP group .
	manualset3
98226	1	400177	5	NULL	NULL	0	NULL	adaptation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there was no adaptation when reaching or looking at an object in the same orientation , suggesting that hand orientation , rather than object orientation , was the critical factor .
	manualset3
98227	2	400177	5	NULL	NULL	0	NULL	object	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there was no adaptation when reaching or looking at an object in the same orientation , suggesting that hand orientation , rather than object orientation , was the critical factor .
	manualset3
98228	3	400177	5	NULL	NULL	0	NULL	 same orientation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there was no adaptation when reaching or looking at an object in the same orientation , suggesting that hand orientation , rather than object orientation , was the critical factor .
	manualset3
98229	4	400177	5	NULL	NULL	0	NULL	hand orientation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there was no adaptation when reaching or looking at an object in the same orientation , suggesting that hand orientation , rather than object orientation , was the critical factor .
	manualset3
98230	5	400177	5	NULL	NULL	0	NULL	object orientation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there was no adaptation when reaching or looking at an object in the same orientation , suggesting that hand orientation , rather than object orientation , was the critical factor .
	manualset3
98231	6	400177	5	NULL	NULL	0	NULL	critical factor	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there was no adaptation when reaching or looking at an object in the same orientation , suggesting that hand orientation , rather than object orientation , was the critical factor .
	manualset3
98232	1	400178	5	NULL	NULL	0	NULL	bulk	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there was no appreciable decrease in the bulk of other plasma proteins , such as various transport proteins ( albumin , prealbumin , transferrin ) and immunoglobulins , during 4 h of incubation with the bacterium .
	manualset3
98233	2	400178	5	NULL	NULL	0	NULL	plasma proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there was no appreciable decrease in the bulk of other plasma proteins , such as various transport proteins ( albumin , prealbumin , transferrin ) and immunoglobulins , during 4 h of incubation with the bacterium .
	manualset3
98234	3	400178	5	NULL	NULL	NULL	NULL	various transport proteins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , there was no appreciable decrease in the bulk of other plasma proteins , such as various transport proteins ( albumin , prealbumin , transferrin ) and immunoglobulins , during 4 h of incubation with the bacterium .
	manualset3
98235	4	400178	5	NULL	NULL	0	NULL	albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there was no appreciable decrease in the bulk of other plasma proteins , such as various transport proteins ( albumin , prealbumin , transferrin ) and immunoglobulins , during 4 h of incubation with the bacterium .
	manualset3
98236	5	400178	5	NULL	NULL	0	NULL	prealbumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there was no appreciable decrease in the bulk of other plasma proteins , such as various transport proteins ( albumin , prealbumin , transferrin ) and immunoglobulins , during 4 h of incubation with the bacterium .
	manualset3
98237	6	400178	5	NULL	NULL	0	NULL	transferrin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there was no appreciable decrease in the bulk of other plasma proteins , such as various transport proteins ( albumin , prealbumin , transferrin ) and immunoglobulins , during 4 h of incubation with the bacterium .
	manualset3
98238	7	400178	5	NULL	NULL	0	NULL	immunoglobulins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there was no appreciable decrease in the bulk of other plasma proteins , such as various transport proteins ( albumin , prealbumin , transferrin ) and immunoglobulins , during 4 h of incubation with the bacterium .
	manualset3
98239	8	400178	5	NULL	NULL	0	NULL	4 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there was no appreciable decrease in the bulk of other plasma proteins , such as various transport proteins ( albumin , prealbumin , transferrin ) and immunoglobulins , during 4 h of incubation with the bacterium .
	manualset3
98240	9	400178	5	NULL	NULL	0	NULL	incubation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there was no appreciable decrease in the bulk of other plasma proteins , such as various transport proteins ( albumin , prealbumin , transferrin ) and immunoglobulins , during 4 h of incubation with the bacterium .
	manualset3
98241	10	400178	5	NULL	NULL	0	NULL	bacterium	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there was no appreciable decrease in the bulk of other plasma proteins , such as various transport proteins ( albumin , prealbumin , transferrin ) and immunoglobulins , during 4 h of incubation with the bacterium .
	manualset3
98242	1	400179	5	NULL	NULL	0	NULL	false-positive results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there were no false-positive results using an anti-mu capture method , even in sera from cases of infectious mononucleosis .
	manualset3
98243	2	400179	5	NULL	NULL	0	NULL	anti-mu capture method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there were no false-positive results using an anti-mu capture method , even in sera from cases of infectious mononucleosis .
	manualset3
98244	3	400179	5	NULL	NULL	0	NULL	sera	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there were no false-positive results using an anti-mu capture method , even in sera from cases of infectious mononucleosis .
	manualset3
98245	4	400179	5	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there were no false-positive results using an anti-mu capture method , even in sera from cases of infectious mononucleosis .
	manualset3
98246	5	400179	5	NULL	NULL	0	NULL	infectious mononucleosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , there were no false-positive results using an anti-mu capture method , even in sera from cases of infectious mononucleosis .
	manualset3
98247	1	400180	5	NULL	NULL	0	NULL	thrombin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , thrombin had no effect on eosinophil function .
	manualset3
98248	2	400180	5	NULL	NULL	0	NULL	eosinophil function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , thrombin had no effect on eosinophil function .
	manualset3
98249	1	400181	5	NULL	NULL	0	NULL	total levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , total levels of - internexin and binding of - internexin to the spinophilin N-terminal domain increases with maturation , perhaps bridging an indirect interaction with CaMKII .
	manualset3
98250	2	400181	5	NULL	NULL	0	NULL	internexin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , total levels of - internexin and binding of - internexin to the spinophilin N-terminal domain increases with maturation , perhaps bridging an indirect interaction with CaMKII .
	manualset3
98251	3	400181	5	NULL	NULL	0	NULL	internexin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , total levels of - internexin and binding of - internexin to the spinophilin N-terminal domain increases with maturation , perhaps bridging an indirect interaction with CaMKII .
	manualset3
98252	4	400181	5	NULL	NULL	0	NULL	spinophilin N-terminal domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , total levels of - internexin and binding of - internexin to the spinophilin N-terminal domain increases with maturation , perhaps bridging an indirect interaction with CaMKII .
	manualset3
98253	5	400181	5	NULL	NULL	0	NULL	maturation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , total levels of - internexin and binding of - internexin to the spinophilin N-terminal domain increases with maturation , perhaps bridging an indirect interaction with CaMKII .
	manualset3
98254	6	400181	5	NULL	NULL	0	NULL	indirect interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , total levels of - internexin and binding of - internexin to the spinophilin N-terminal domain increases with maturation , perhaps bridging an indirect interaction with CaMKII .
	manualset3
98255	7	400181	5	NULL	NULL	0	NULL	CaMKII	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , total levels of - internexin and binding of - internexin to the spinophilin N-terminal domain increases with maturation , perhaps bridging an indirect interaction with CaMKII .
	manualset3
98256	1	400182	5	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , treatment of depression and the influence of treatment on outcomes have been studied to some extent .
	manualset3
98257	2	400182	5	NULL	NULL	0	NULL	depression	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , treatment of depression and the influence of treatment on outcomes have been studied to some extent .
	manualset3
98258	3	400182	5	NULL	NULL	NULL	NULL	influence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , treatment of depression and the influence of treatment on outcomes have been studied to some extent .
	manualset3
98259	4	400182	5	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , treatment of depression and the influence of treatment on outcomes have been studied to some extent .
	manualset3
98260	5	400182	5	NULL	NULL	0	NULL	outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , treatment of depression and the influence of treatment on outcomes have been studied to some extent .
	manualset3
98261	1	400183	5	NULL	NULL	0	NULL	u-PA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , u-PA bound to endogenously occupied receptors is inhibited by PAI-2 only at PAI : u-PA molar ratios of 20 : 1 , but is not inhibited by PAI-1 , u-PA/PAI -1 and u-PA/PAI -2 complexes bind to the receptor with a tenfold lower affinity than u-PA itself .
	manualset3
98262	2	400183	5	NULL	NULL	0	NULL	endogenously occupied receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , u-PA bound to endogenously occupied receptors is inhibited by PAI-2 only at PAI : u-PA molar ratios of 20 : 1 , but is not inhibited by PAI-1 , u-PA/PAI -1 and u-PA/PAI -2 complexes bind to the receptor with a tenfold lower affinity than u-PA itself .
	manualset3
98263	3	400183	5	NULL	NULL	0	NULL	PAI-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , u-PA bound to endogenously occupied receptors is inhibited by PAI-2 only at PAI : u-PA molar ratios of 20 : 1 , but is not inhibited by PAI-1 , u-PA/PAI -1 and u-PA/PAI -2 complexes bind to the receptor with a tenfold lower affinity than u-PA itself .
	manualset3
98264	4	400183	5	NULL	NULL	0	NULL	PAI : u-PA molar ratios	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , u-PA bound to endogenously occupied receptors is inhibited by PAI-2 only at PAI : u-PA molar ratios of 20 : 1 , but is not inhibited by PAI-1 , u-PA/PAI -1 and u-PA/PAI -2 complexes bind to the receptor with a tenfold lower affinity than u-PA itself .
	manualset3
98265	5	400183	5	NULL	NULL	0	NULL	20 : 1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , u-PA bound to endogenously occupied receptors is inhibited by PAI-2 only at PAI : u-PA molar ratios of 20 : 1 , but is not inhibited by PAI-1 , u-PA/PAI -1 and u-PA/PAI -2 complexes bind to the receptor with a tenfold lower affinity than u-PA itself .
	manualset3
98266	6	400183	5	NULL	NULL	0	NULL	PAI-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , u-PA bound to endogenously occupied receptors is inhibited by PAI-2 only at PAI : u-PA molar ratios of 20 : 1 , but is not inhibited by PAI-1 , u-PA/PAI -1 and u-PA/PAI -2 complexes bind to the receptor with a tenfold lower affinity than u-PA itself .
	manualset3
98267	7	400183	5	NULL	NULL	0	NULL	u-PA/PAI -1 complex	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , u-PA bound to endogenously occupied receptors is inhibited by PAI-2 only at PAI : u-PA molar ratios of 20 : 1 , but is not inhibited by PAI-1 , u-PA/PAI -1 and u-PA/PAI -2 complexes bind to the receptor with a tenfold lower affinity than u-PA itself .
	manualset3
98268	8	400183	5	NULL	NULL	0	NULL	u-PA/PAI -2 complex	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , u-PA bound to endogenously occupied receptors is inhibited by PAI-2 only at PAI : u-PA molar ratios of 20 : 1 , but is not inhibited by PAI-1 , u-PA/PAI -1 and u-PA/PAI -2 complexes bind to the receptor with a tenfold lower affinity than u-PA itself .
	manualset3
98269	9	400183	5	NULL	NULL	0	NULL	receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , u-PA bound to endogenously occupied receptors is inhibited by PAI-2 only at PAI : u-PA molar ratios of 20 : 1 , but is not inhibited by PAI-1 , u-PA/PAI -1 and u-PA/PAI -2 complexes bind to the receptor with a tenfold lower affinity than u-PA itself .
	manualset3
98270	10	400183	5	NULL	NULL	NULL	NULL	 tenfold lower affinity	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , u-PA bound to endogenously occupied receptors is inhibited by PAI-2 only at PAI : u-PA molar ratios of 20 : 1 , but is not inhibited by PAI-1 , u-PA/PAI -1 and u-PA/PAI -2 complexes bind to the receptor with a tenfold lower affinity than u-PA itself .
	manualset3
98271	11	400183	5	NULL	NULL	0	NULL	u-PA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , u-PA bound to endogenously occupied receptors is inhibited by PAI-2 only at PAI : u-PA molar ratios of 20 : 1 , but is not inhibited by PAI-1 , u-PA/PAI -1 and u-PA/PAI -2 complexes bind to the receptor with a tenfold lower affinity than u-PA itself .
	manualset3
98272	1	400184	5	NULL	NULL	0	NULL	susceptibility 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , very little is known about the susceptibility of developing germ cells to apoptosis in response to busulfan treatment .
	manualset3
98273	2	400184	5	NULL	NULL	0	NULL	germ cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , very little is known about the susceptibility of developing germ cells to apoptosis in response to busulfan treatment .
	manualset3
98274	3	400184	5	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , very little is known about the susceptibility of developing germ cells to apoptosis in response to busulfan treatment .
	manualset3
98275	4	400184	5	NULL	NULL	0	NULL	response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , very little is known about the susceptibility of developing germ cells to apoptosis in response to busulfan treatment .
	manualset3
98276	5	400184	5	NULL	NULL	0	NULL	busulfan treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , very little is known about the susceptibility of developing germ cells to apoptosis in response to busulfan treatment .
	manualset3
98277	1	400185	5	NULL	NULL	0	NULL	work	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , very little work in this area has been done on herbicide metabolites in soil .
	manualset3
98278	2	400185	5	NULL	NULL	0	NULL	area	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , very little work in this area has been done on herbicide metabolites in soil .
	manualset3
98279	3	400185	5	NULL	NULL	0	NULL	herbicide metabolites	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , very little work in this area has been done on herbicide metabolites in soil .
	manualset3
98280	4	400185	5	NULL	NULL	0	NULL	soil	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , very little work in this area has been done on herbicide metabolites in soil .
	manualset3
98281	1	400186	5	NULL	NULL	0	NULL	buried and surface water 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , we find that both the buried and surface water are entropically unfavored : buried water is 0.9-2 .2 kcal/mol lower than the bulk while the surface water is 0.1-0 .2 kcal/mol lower .
	manualset3
98282	2	400186	5	NULL	NULL	0	NULL	 buried water 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , we find that both the buried and surface water are entropically unfavored : buried water is 0.9-2 .2 kcal/mol lower than the bulk while the surface water is 0.1-0 .2 kcal/mol lower .
	manualset3
98283	3	400186	5	NULL	NULL	0	NULL	0.9-2 .2 kcal/mol	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , we find that both the buried and surface water are entropically unfavored : buried water is 0.9-2 .2 kcal/mol lower than the bulk while the surface water is 0.1-0 .2 kcal/mol lower .
	manualset3
98284	4	400186	5	NULL	NULL	0	NULL	bulk	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , we find that both the buried and surface water are entropically unfavored : buried water is 0.9-2 .2 kcal/mol lower than the bulk while the surface water is 0.1-0 .2 kcal/mol lower .
	manualset3
98285	5	400186	5	NULL	NULL	0	NULL	surface water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , we find that both the buried and surface water are entropically unfavored : buried water is 0.9-2 .2 kcal/mol lower than the bulk while the surface water is 0.1-0 .2 kcal/mol lower .
	manualset3
98286	6	400186	5	NULL	NULL	0	NULL	0.1-0 .2 kcal/mol	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , we find that both the buried and surface water are entropically unfavored : buried water is 0.9-2 .2 kcal/mol lower than the bulk while the surface water is 0.1-0 .2 kcal/mol lower .
	manualset3
98287	1	400187	5	NULL	NULL	0	NULL	drug trial	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Why has the drug trial at Northwick Park Hospital turned out to a disaster ? ) .
	manualset3
98288	2	400187	5	NULL	NULL	0	NULL	Northwick Park Hospital	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( Why has the drug trial at Northwick Park Hospital turned out to a disaster ? ) .
	manualset3
98289	3	400187	5	NULL	NULL	0	NULL	disaster	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Why has the drug trial at Northwick Park Hospital turned out to a disaster ? ) .
	manualset3
98290	1	400188	5	NULL	NULL	0	NULL	lower sensitivity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , we observed lower sensitivity to quinolinic acid in spite of unaltered glutamate uptake by the same cerebral structures .
	manualset3
98291	2	400188	5	NULL	NULL	0	NULL	quinolinic acid	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , we observed lower sensitivity to quinolinic acid in spite of unaltered glutamate uptake by the same cerebral structures .
	manualset3
98292	3	400188	5	NULL	NULL	0	NULL	unaltered glutamate uptake	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , we observed lower sensitivity to quinolinic acid in spite of unaltered glutamate uptake by the same cerebral structures .
	manualset3
98293	4	400188	5	NULL	NULL	0	NULL	cerebral structures	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , we observed lower sensitivity to quinolinic acid in spite of unaltered glutamate uptake by the same cerebral structures .
	manualset3
98294	1	400189	5	NULL	NULL	0	NULL	administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , while administration of MA has been reported to stimulate food intake in pre-pubertal female rats , food intake is not stimulated by MA in adult female rats .
	manualset3
98295	2	400189	5	NULL	NULL	0	NULL	MA	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , while administration of MA has been reported to stimulate food intake in pre-pubertal female rats , food intake is not stimulated by MA in adult female rats .
	manualset3
98296	3	400189	5	NULL	NULL	0	NULL	food intake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , while administration of MA has been reported to stimulate food intake in pre-pubertal female rats , food intake is not stimulated by MA in adult female rats .
	manualset3
98297	4	400189	5	NULL	NULL	0	NULL	pre-pubertal female rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , while administration of MA has been reported to stimulate food intake in pre-pubertal female rats , food intake is not stimulated by MA in adult female rats .
	manualset3
98298	5	400189	5	NULL	NULL	0	NULL	food intake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , while administration of MA has been reported to stimulate food intake in pre-pubertal female rats , food intake is not stimulated by MA in adult female rats .
	manualset3
98299	6	400189	5	NULL	NULL	0	NULL	MA	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , while administration of MA has been reported to stimulate food intake in pre-pubertal female rats , food intake is not stimulated by MA in adult female rats .
	manualset3
98300	7	400189	5	NULL	NULL	0	NULL	adult female rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , while administration of MA has been reported to stimulate food intake in pre-pubertal female rats , food intake is not stimulated by MA in adult female rats .
	manualset3
98301	1	400190	5	NULL	NULL	0	NULL	ankyrin , protein band 3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast ankyrin , protein band 3 and protein 4.2 are removed from skeletons as the ionic strength increased .
	manualset3
98302	2	400190	5	NULL	NULL	0	NULL	ankyrin , protein 4.2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast ankyrin , protein band 3 and protein 4.2 are removed from skeletons as the ionic strength increased .
	manualset3
98303	3	400190	5	NULL	NULL	0	NULL	skeletons	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast ankyrin , protein band 3 and protein 4.2 are removed from skeletons as the ionic strength increased .
	manualset3
98304	4	400190	5	NULL	NULL	0	NULL	ionic strength	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast ankyrin , protein band 3 and protein 4.2 are removed from skeletons as the ionic strength increased .
	manualset3
98305	1	400191	5	NULL	NULL	NULL	NULL	umuC mutation	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast the umuC mutation does not significantly affect the induction kinetics .
	manualset3
98306	2	400191	5	NULL	NULL	0	NULL	induction kinetics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast the umuC mutation does not significantly affect the induction kinetics .
	manualset3
98307	1	400192	5	NULL	NULL	0	NULL	Bf 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to Bf and C2 , each of which is coded for by codominant alleles at a single genetic locus , C4 is coded for by two genes , C4F ( Rodgers ) and C4S ( Chido ) .
	manualset3
98308	2	400192	5	NULL	NULL	0	NULL	C2	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to Bf and C2 , each of which is coded for by codominant alleles at a single genetic locus , C4 is coded for by two genes , C4F ( Rodgers ) and C4S ( Chido ) .
	manualset3
98309	3	400192	5	NULL	NULL	0	NULL	codominant alleles	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to Bf and C2 , each of which is coded for by codominant alleles at a single genetic locus , C4 is coded for by two genes , C4F ( Rodgers ) and C4S ( Chido ) .
	manualset3
98310	4	400192	5	NULL	NULL	0	NULL	single genetic locus	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to Bf and C2 , each of which is coded for by codominant alleles at a single genetic locus , C4 is coded for by two genes , C4F ( Rodgers ) and C4S ( Chido ) .
	manualset3
98311	5	400192	5	NULL	NULL	0	NULL	C4	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to Bf and C2 , each of which is coded for by codominant alleles at a single genetic locus , C4 is coded for by two genes , C4F ( Rodgers ) and C4S ( Chido ) .
	manualset3
98312	6	400192	5	NULL	NULL	0	NULL	two genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to Bf and C2 , each of which is coded for by codominant alleles at a single genetic locus , C4 is coded for by two genes , C4F ( Rodgers ) and C4S ( Chido ) .
	manualset3
98313	7	400192	5	NULL	NULL	0	NULL	C4F ( Rodgers )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to Bf and C2 , each of which is coded for by codominant alleles at a single genetic locus , C4 is coded for by two genes , C4F ( Rodgers ) and C4S ( Chido ) .
	manualset3
98314	8	400192	5	NULL	NULL	0	NULL	C4S ( Chido )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to Bf and C2 , each of which is coded for by codominant alleles at a single genetic locus , C4 is coded for by two genes , C4F ( Rodgers ) and C4S ( Chido ) .
	manualset3
98315	1	400193	5	NULL	NULL	0	NULL	DHEA	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to DHEA and EpiA , the 7-hydroxylated derivatives were shown to mediate neuroprotection , and 7beta-hydroxy-EpiA was the most potent .
	manualset3
98316	2	400193	5	NULL	NULL	0	NULL	EpiA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to DHEA and EpiA , the 7-hydroxylated derivatives were shown to mediate neuroprotection , and 7beta-hydroxy-EpiA was the most potent .
	manualset3
98317	3	400193	5	NULL	NULL	0	NULL	7-hydroxylated derivatives	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to DHEA and EpiA , the 7-hydroxylated derivatives were shown to mediate neuroprotection , and 7beta-hydroxy-EpiA was the most potent .
	manualset3
98318	4	400193	5	NULL	NULL	0	NULL	neuroprotection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to DHEA and EpiA , the 7-hydroxylated derivatives were shown to mediate neuroprotection , and 7beta-hydroxy-EpiA was the most potent .
	manualset3
98319	5	400193	5	NULL	NULL	0	NULL	7beta-hydroxy-EpiA	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to DHEA and EpiA , the 7-hydroxylated derivatives were shown to mediate neuroprotection , and 7beta-hydroxy-EpiA was the most potent .
	manualset3
98320	1	400194	5	NULL	NULL	0	NULL	PIM	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to PIM , use of common virtual oscillatory centroids enabled the FSCA to reveal multiple dynamical neural assemblies as well as the unitary phase information within each assembly .
	manualset3
98321	2	400194	5	NULL	NULL	NULL	NULL	virtual oscillatory centroids	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast to PIM , use of common virtual oscillatory centroids enabled the FSCA to reveal multiple dynamical neural assemblies as well as the unitary phase information within each assembly .
	manualset3
98322	3	400194	5	NULL	NULL	0	NULL	FSCA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to PIM , use of common virtual oscillatory centroids enabled the FSCA to reveal multiple dynamical neural assemblies as well as the unitary phase information within each assembly .
	manualset3
98323	4	400194	5	NULL	NULL	0	NULL	multiple dynamical neural assemblies	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to PIM , use of common virtual oscillatory centroids enabled the FSCA to reveal multiple dynamical neural assemblies as well as the unitary phase information within each assembly .
	manualset3
98324	5	400194	5	NULL	NULL	0	NULL	unitary phase information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to PIM , use of common virtual oscillatory centroids enabled the FSCA to reveal multiple dynamical neural assemblies as well as the unitary phase information within each assembly .
	manualset3
98325	6	400194	5	NULL	NULL	0	NULL	assembly	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to PIM , use of common virtual oscillatory centroids enabled the FSCA to reveal multiple dynamical neural assemblies as well as the unitary phase information within each assembly .
	manualset3
98326	1	400195	5	NULL	NULL	0	NULL	Tg ( IL1 ) mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to Tg ( IL1 ) mice , pancreatitis was significantly less severe in dual-transgenic ( Tg ( IL1 ) - Tg ( Psti1 ) ) mice expressing IL-1 and PSTI-I in pancreatic acinar cells .
	manualset3
98327	2	400195	5	NULL	NULL	0	NULL	pancreatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to Tg ( IL1 ) mice , pancreatitis was significantly less severe in dual-transgenic ( Tg ( IL1 ) - Tg ( Psti1 ) ) mice expressing IL-1 and PSTI-I in pancreatic acinar cells .
	manualset3
98328	3	400195	5	NULL	NULL	0	NULL	dual-transgenic ( Tg ( IL1 ) - Tg ( Psti1 ) ) mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to Tg ( IL1 ) mice , pancreatitis was significantly less severe in dual-transgenic ( Tg ( IL1 ) - Tg ( Psti1 ) ) mice expressing IL-1 and PSTI-I in pancreatic acinar cells .
	manualset3
98329	4	400195	5	NULL	NULL	0	NULL	IL-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to Tg ( IL1 ) mice , pancreatitis was significantly less severe in dual-transgenic ( Tg ( IL1 ) - Tg ( Psti1 ) ) mice expressing IL-1 and PSTI-I in pancreatic acinar cells .
	manualset3
98330	5	400195	5	NULL	NULL	0	NULL	PSTI-I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to Tg ( IL1 ) mice , pancreatitis was significantly less severe in dual-transgenic ( Tg ( IL1 ) - Tg ( Psti1 ) ) mice expressing IL-1 and PSTI-I in pancreatic acinar cells .
	manualset3
98331	6	400195	5	NULL	NULL	0	NULL	pancreatic acinar cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to Tg ( IL1 ) mice , pancreatitis was significantly less severe in dual-transgenic ( Tg ( IL1 ) - Tg ( Psti1 ) ) mice expressing IL-1 and PSTI-I in pancreatic acinar cells .
	manualset3
98332	1	400196	5	NULL	NULL	NULL	NULL	Thiomargarita namibiensis populations	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast to Thiomargarita namibiensis populations , which rely on periodic resuspension from sulfidic sediment into the oxygenated water column , Thiomargarita cells at the Amon mud volcano seem to remain stationary at the sediment surface while environmental conditions change around them due to periodic brine flow .
	manualset3
98333	2	400196	5	NULL	NULL	0	NULL	periodic resuspension	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to Thiomargarita namibiensis populations , which rely on periodic resuspension from sulfidic sediment into the oxygenated water column , Thiomargarita cells at the Amon mud volcano seem to remain stationary at the sediment surface while environmental conditions change around them due to periodic brine flow .
	manualset3
98334	3	400196	5	NULL	NULL	NULL	NULL	sulfidic sediment	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast to Thiomargarita namibiensis populations , which rely on periodic resuspension from sulfidic sediment into the oxygenated water column , Thiomargarita cells at the Amon mud volcano seem to remain stationary at the sediment surface while environmental conditions change around them due to periodic brine flow .
	manualset3
98335	4	400196	5	NULL	NULL	NULL	NULL	oxygenated water column	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast to Thiomargarita namibiensis populations , which rely on periodic resuspension from sulfidic sediment into the oxygenated water column , Thiomargarita cells at the Amon mud volcano seem to remain stationary at the sediment surface while environmental conditions change around them due to periodic brine flow .
	manualset3
98336	5	400196	5	NULL	NULL	0	NULL	Thiomargarita cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to Thiomargarita namibiensis populations , which rely on periodic resuspension from sulfidic sediment into the oxygenated water column , Thiomargarita cells at the Amon mud volcano seem to remain stationary at the sediment surface while environmental conditions change around them due to periodic brine flow .
	manualset3
98337	6	400196	5	NULL	NULL	0	NULL	Amon mud volcano	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to Thiomargarita namibiensis populations , which rely on periodic resuspension from sulfidic sediment into the oxygenated water column , Thiomargarita cells at the Amon mud volcano seem to remain stationary at the sediment surface while environmental conditions change around them due to periodic brine flow .
	manualset3
98338	7	400196	5	NULL	NULL	0	NULL	sediment surface	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to Thiomargarita namibiensis populations , which rely on periodic resuspension from sulfidic sediment into the oxygenated water column , Thiomargarita cells at the Amon mud volcano seem to remain stationary at the sediment surface while environmental conditions change around them due to periodic brine flow .
	manualset3
98339	8	400196	5	NULL	NULL	0	NULL	environmental conditions	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to Thiomargarita namibiensis populations , which rely on periodic resuspension from sulfidic sediment into the oxygenated water column , Thiomargarita cells at the Amon mud volcano seem to remain stationary at the sediment surface while environmental conditions change around them due to periodic brine flow .
	manualset3
98340	9	400196	5	NULL	NULL	0	NULL	periodic brine flow	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to Thiomargarita namibiensis populations , which rely on periodic resuspension from sulfidic sediment into the oxygenated water column , Thiomargarita cells at the Amon mud volcano seem to remain stationary at the sediment surface while environmental conditions change around them due to periodic brine flow .
	manualset3
98341	1	400197	5	NULL	NULL	0	NULL	Work	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Work , violence and death in Campinas , So Paulo , Brazil ) .
	manualset3
98342	2	400197	5	NULL	NULL	0	NULL	violence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Work , violence and death in Campinas , So Paulo , Brazil ) .
	manualset3
98343	3	400197	5	NULL	NULL	0	NULL	death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Work , violence and death in Campinas , So Paulo , Brazil ) .
	manualset3
98344	4	400197	5	NULL	NULL	0	NULL	Campinas , So Paulo , Brazil	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Work , violence and death in Campinas , So Paulo , Brazil ) .
	manualset3
98345	1	400198	5	NULL	NULL	0	NULL	VIP	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to VIP , the prevalence rate did not affect costs for processing pools by EIA .
	manualset3
98346	2	400198	5	NULL	NULL	0	NULL	prevalence rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to VIP , the prevalence rate did not affect costs for processing pools by EIA .
	manualset3
98347	3	400198	5	NULL	NULL	0	NULL	pools	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to VIP , the prevalence rate did not affect costs for processing pools by EIA .
	manualset3
98348	4	400198	5	NULL	NULL	0	NULL	EIA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to VIP , the prevalence rate did not affect costs for processing pools by EIA .
	manualset3
98349	1	400199	5	NULL	NULL	0	NULL	cell injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to cell injection in the nonvitrectomized eye , in which vitreous membranes predominate , this model stresses epiretinal membrane and surface retinal traction .
	manualset3
98350	2	400199	5	NULL	NULL	0	NULL	nonvitrectomized eye	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to cell injection in the nonvitrectomized eye , in which vitreous membranes predominate , this model stresses epiretinal membrane and surface retinal traction .
	manualset3
98351	3	400199	5	NULL	NULL	0	NULL	vitreous membranes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to cell injection in the nonvitrectomized eye , in which vitreous membranes predominate , this model stresses epiretinal membrane and surface retinal traction .
	manualset3
98352	4	400199	5	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to cell injection in the nonvitrectomized eye , in which vitreous membranes predominate , this model stresses epiretinal membrane and surface retinal traction .
	manualset3
98353	5	400199	5	NULL	NULL	0	NULL	epiretinal membrane	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to cell injection in the nonvitrectomized eye , in which vitreous membranes predominate , this model stresses epiretinal membrane and surface retinal traction .
	manualset3
98354	6	400199	5	NULL	NULL	0	NULL	surface retinal traction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to cell injection in the nonvitrectomized eye , in which vitreous membranes predominate , this model stresses epiretinal membrane and surface retinal traction .
	manualset3
98355	1	400200	5	NULL	NULL	0	NULL	chimpanzees	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to chimpanzees previously tested on the same task ( S. T. Boysen & G. G. Berntson , 1995 ; S. T. Boysen , G. G. Berntson , M. B. Hannan , & J. T. Cacioppo , 1996 ; S. T. Boysen , K. L. Mukobi , & G. G. Berntson , 1999 ) , the orangutans optimized their performance .
	manualset3
98356	2	400200	5	NULL	NULL	0	NULL	task 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to chimpanzees previously tested on the same task ( S. T. Boysen & G. G. Berntson , 1995 ; S. T. Boysen , G. G. Berntson , M. B. Hannan , & J. T. Cacioppo , 1996 ; S. T. Boysen , K. L. Mukobi , & G. G. Berntson , 1999 ) , the orangutans optimized their performance .
	manualset3
98357	3	400200	5	NULL	NULL	0	NULL	S. T. Boysen & G. G. Berntson , 1995	Citation												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to chimpanzees previously tested on the same task ( S. T. Boysen & G. G. Berntson , 1995 ; S. T. Boysen , G. G. Berntson , M. B. Hannan , & J. T. Cacioppo , 1996 ; S. T. Boysen , K. L. Mukobi , & G. G. Berntson , 1999 ) , the orangutans optimized their performance .
	manualset3
98358	4	400200	5	NULL	NULL	0	NULL	S. T. Boysen , G. G. Berntson , M. B. Hannan , & J. T. Cacioppo , 1996	Citation												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to chimpanzees previously tested on the same task ( S. T. Boysen & G. G. Berntson , 1995 ; S. T. Boysen , G. G. Berntson , M. B. Hannan , & J. T. Cacioppo , 1996 ; S. T. Boysen , K. L. Mukobi , & G. G. Berntson , 1999 ) , the orangutans optimized their performance .
	manualset3
98359	5	400200	5	NULL	NULL	0	NULL	S. T. Boysen , K. L. Mukobi , & G. G. Berntson , 1999	Citation												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to chimpanzees previously tested on the same task ( S. T. Boysen & G. G. Berntson , 1995 ; S. T. Boysen , G. G. Berntson , M. B. Hannan , & J. T. Cacioppo , 1996 ; S. T. Boysen , K. L. Mukobi , & G. G. Berntson , 1999 ) , the orangutans optimized their performance .
	manualset3
98360	6	400200	5	NULL	NULL	0	NULL	orangutans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to chimpanzees previously tested on the same task ( S. T. Boysen & G. G. Berntson , 1995 ; S. T. Boysen , G. G. Berntson , M. B. Hannan , & J. T. Cacioppo , 1996 ; S. T. Boysen , K. L. Mukobi , & G. G. Berntson , 1999 ) , the orangutans optimized their performance .
	manualset3
98361	7	400200	5	NULL	NULL	0	NULL	performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to chimpanzees previously tested on the same task ( S. T. Boysen & G. G. Berntson , 1995 ; S. T. Boysen , G. G. Berntson , M. B. Hannan , & J. T. Cacioppo , 1996 ; S. T. Boysen , K. L. Mukobi , & G. G. Berntson , 1999 ) , the orangutans optimized their performance .
	manualset3
98362	1	400201	5	NULL	NULL	0	NULL	conventional models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to conventional models of STDP in which spike-timing affects weights of synaptic connections , we consider a model of STDP in which the time lags between pre - and/or post-synaptic spikes change internal state of pre - and/or post-synaptic neurons respectively .
	manualset3
98363	2	400201	5	NULL	NULL	NULL	NULL	STDP	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast to conventional models of STDP in which spike-timing affects weights of synaptic connections , we consider a model of STDP in which the time lags between pre - and/or post-synaptic spikes change internal state of pre - and/or post-synaptic neurons respectively .
	manualset3
98364	3	400201	5	NULL	NULL	0	NULL	spike-timing	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to conventional models of STDP in which spike-timing affects weights of synaptic connections , we consider a model of STDP in which the time lags between pre - and/or post-synaptic spikes change internal state of pre - and/or post-synaptic neurons respectively .
	manualset3
98365	4	400201	5	NULL	NULL	0	NULL	weights	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to conventional models of STDP in which spike-timing affects weights of synaptic connections , we consider a model of STDP in which the time lags between pre - and/or post-synaptic spikes change internal state of pre - and/or post-synaptic neurons respectively .
	manualset3
98366	5	400201	5	NULL	NULL	0	NULL	synaptic connections	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to conventional models of STDP in which spike-timing affects weights of synaptic connections , we consider a model of STDP in which the time lags between pre - and/or post-synaptic spikes change internal state of pre - and/or post-synaptic neurons respectively .
	manualset3
98367	6	400201	5	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to conventional models of STDP in which spike-timing affects weights of synaptic connections , we consider a model of STDP in which the time lags between pre - and/or post-synaptic spikes change internal state of pre - and/or post-synaptic neurons respectively .
	manualset3
98368	7	400201	5	NULL	NULL	0	NULL	STDP	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to conventional models of STDP in which spike-timing affects weights of synaptic connections , we consider a model of STDP in which the time lags between pre - and/or post-synaptic spikes change internal state of pre - and/or post-synaptic neurons respectively .
	manualset3
98369	8	400201	5	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to conventional models of STDP in which spike-timing affects weights of synaptic connections , we consider a model of STDP in which the time lags between pre - and/or post-synaptic spikes change internal state of pre - and/or post-synaptic neurons respectively .
	manualset3
98370	9	400201	5	NULL	NULL	0	NULL	pre - and/or post-synaptic spikes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to conventional models of STDP in which spike-timing affects weights of synaptic connections , we consider a model of STDP in which the time lags between pre - and/or post-synaptic spikes change internal state of pre - and/or post-synaptic neurons respectively .
	manualset3
98371	10	400201	5	NULL	NULL	0	NULL	internal state	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to conventional models of STDP in which spike-timing affects weights of synaptic connections , we consider a model of STDP in which the time lags between pre - and/or post-synaptic spikes change internal state of pre - and/or post-synaptic neurons respectively .
	manualset3
98372	11	400201	5	NULL	NULL	0	NULL	pre - and/or post-synaptic neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to conventional models of STDP in which spike-timing affects weights of synaptic connections , we consider a model of STDP in which the time lags between pre - and/or post-synaptic spikes change internal state of pre - and/or post-synaptic neurons respectively .
	manualset3
98373	1	400202	5	NULL	NULL	0	NULL	intact cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to intact cells , purified uPA receptor ( isolated from phorbol 12-myristate 13-acetate-stimulated U937 cells ) was observed to partially inhibit uPA-catalyzed Plg activation , although activity against low molecular weight substrates was retained .
	manualset3
98374	2	400202	5	NULL	NULL	0	NULL	purified uPA receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to intact cells , purified uPA receptor ( isolated from phorbol 12-myristate 13-acetate-stimulated U937 cells ) was observed to partially inhibit uPA-catalyzed Plg activation , although activity against low molecular weight substrates was retained .
	manualset3
98375	3	400202	5	NULL	NULL	0	NULL	phorbol 12-myristate 13-acetate-stimulated U937 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to intact cells , purified uPA receptor ( isolated from phorbol 12-myristate 13-acetate-stimulated U937 cells ) was observed to partially inhibit uPA-catalyzed Plg activation , although activity against low molecular weight substrates was retained .
	manualset3
98376	4	400202	5	NULL	NULL	0	NULL	uPA-catalyzed Plg activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to intact cells , purified uPA receptor ( isolated from phorbol 12-myristate 13-acetate-stimulated U937 cells ) was observed to partially inhibit uPA-catalyzed Plg activation , although activity against low molecular weight substrates was retained .
	manualset3
98377	5	400202	5	NULL	NULL	0	NULL	activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to intact cells , purified uPA receptor ( isolated from phorbol 12-myristate 13-acetate-stimulated U937 cells ) was observed to partially inhibit uPA-catalyzed Plg activation , although activity against low molecular weight substrates was retained .
	manualset3
98378	6	400202	5	NULL	NULL	0	NULL	low molecular weight substrates	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to intact cells , purified uPA receptor ( isolated from phorbol 12-myristate 13-acetate-stimulated U937 cells ) was observed to partially inhibit uPA-catalyzed Plg activation , although activity against low molecular weight substrates was retained .
	manualset3
98379	1	400203	5	NULL	NULL	0	NULL	leukemic cells of B-cell lineage	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to leukemic cells of B-cell lineage ( as in B-cell acute or chronic lymphocytic leukemia and non-T-cell , non-B-cell acute lymphocytic leukemia ) , T-cell-leukemia cells responded within five minutes to hypotonic swelling with an increase in potassium permeability and restoration toward isotonic volume .
	manualset3
98380	2	400203	5	NULL	NULL	NULL	NULL	B-cell acute or chronic lymphocytic leukemia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast to leukemic cells of B-cell lineage ( as in B-cell acute or chronic lymphocytic leukemia and non-T-cell , non-B-cell acute lymphocytic leukemia ) , T-cell-leukemia cells responded within five minutes to hypotonic swelling with an increase in potassium permeability and restoration toward isotonic volume .
	manualset3
98382	3	400203	5	NULL	NULL	NULL	NULL	non-T-cell, non-B-cell acute lymphocytic leukemia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast to leukemic cells of B-cell lineage ( as in B-cell acute or chronic lymphocytic leukemia and non-T-cell , non-B-cell acute lymphocytic leukemia ) , T-cell-leukemia cells responded within five minutes to hypotonic swelling with an increase in potassium permeability and restoration toward isotonic volume .
	manualset3
98383	4	400203	5	NULL	NULL	NULL	NULL	T-cell-leukemia cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast to leukemic cells of B-cell lineage ( as in B-cell acute or chronic lymphocytic leukemia and non-T-cell , non-B-cell acute lymphocytic leukemia ) , T-cell-leukemia cells responded within five minutes to hypotonic swelling with an increase in potassium permeability and restoration toward isotonic volume .
	manualset3
98384	5	400203	5	NULL	NULL	NULL	NULL	five minutes	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast to leukemic cells of B-cell lineage ( as in B-cell acute or chronic lymphocytic leukemia and non-T-cell , non-B-cell acute lymphocytic leukemia ) , T-cell-leukemia cells responded within five minutes to hypotonic swelling with an increase in potassium permeability and restoration toward isotonic volume .
	manualset3
98385	6	400203	5	NULL	NULL	NULL	NULL	hypotonic swelling 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast to leukemic cells of B-cell lineage ( as in B-cell acute or chronic lymphocytic leukemia and non-T-cell , non-B-cell acute lymphocytic leukemia ) , T-cell-leukemia cells responded within five minutes to hypotonic swelling with an increase in potassium permeability and restoration toward isotonic volume .
	manualset3
98386	7	400203	5	NULL	NULL	NULL	NULL	potassium permeability	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast to leukemic cells of B-cell lineage ( as in B-cell acute or chronic lymphocytic leukemia and non-T-cell , non-B-cell acute lymphocytic leukemia ) , T-cell-leukemia cells responded within five minutes to hypotonic swelling with an increase in potassium permeability and restoration toward isotonic volume .
	manualset3
98387	8	400203	5	NULL	NULL	NULL	NULL	restoration	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast to leukemic cells of B-cell lineage ( as in B-cell acute or chronic lymphocytic leukemia and non-T-cell , non-B-cell acute lymphocytic leukemia ) , T-cell-leukemia cells responded within five minutes to hypotonic swelling with an increase in potassium permeability and restoration toward isotonic volume .
	manualset3
98388	9	400203	5	NULL	NULL	NULL	NULL	isotonic volume	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast to leukemic cells of B-cell lineage ( as in B-cell acute or chronic lymphocytic leukemia and non-T-cell , non-B-cell acute lymphocytic leukemia ) , T-cell-leukemia cells responded within five minutes to hypotonic swelling with an increase in potassium permeability and restoration toward isotonic volume .
	manualset3
98389	1	400204	5	NULL	NULL	NULL	NULL	non-selective beta-blocking drugs	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast to many non-selective beta-blocking drugs , carvedilol has a more favourable hemodynamic profile , and its lack of adverse influence on the plasma lipid profile may be important in its long-term use .
	manualset3
98390	2	400204	5	NULL	NULL	0	NULL	carvedilol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to many non-selective beta-blocking drugs , carvedilol has a more favourable hemodynamic profile , and its lack of adverse influence on the plasma lipid profile may be important in its long-term use .
	manualset3
98391	3	400204	5	NULL	NULL	0	NULL	favourable hemodynamic profile	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to many non-selective beta-blocking drugs , carvedilol has a more favourable hemodynamic profile , and its lack of adverse influence on the plasma lipid profile may be important in its long-term use .
	manualset3
98392	4	400204	5	NULL	NULL	0	NULL	adverse influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to many non-selective beta-blocking drugs , carvedilol has a more favourable hemodynamic profile , and its lack of adverse influence on the plasma lipid profile may be important in its long-term use .
	manualset3
98393	5	400204	5	NULL	NULL	0	NULL	plasma lipid profile	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to many non-selective beta-blocking drugs , carvedilol has a more favourable hemodynamic profile , and its lack of adverse influence on the plasma lipid profile may be important in its long-term use .
	manualset3
98394	6	400204	5	NULL	NULL	0	NULL	long-term use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to many non-selective beta-blocking drugs , carvedilol has a more favourable hemodynamic profile , and its lack of adverse influence on the plasma lipid profile may be important in its long-term use .
	manualset3
98395	1	400205	5	NULL	NULL	0	NULL	mixotrophic conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to mixotrophic conditions ( up to 80 % contribution ) , cyclic electron transport plays only a minor role ( below 10 % ) under photoautotrophic conditions for all the strains , while linear electron transport increased up to 5.5-fold from WT to PAL mutant .
	manualset3
98396	2	400205	5	NULL	NULL	0	NULL	80 % contribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to mixotrophic conditions ( up to 80 % contribution ) , cyclic electron transport plays only a minor role ( below 10 % ) under photoautotrophic conditions for all the strains , while linear electron transport increased up to 5.5-fold from WT to PAL mutant .
	manualset3
98397	3	400205	5	NULL	NULL	0	NULL	cyclic electron transport	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to mixotrophic conditions ( up to 80 % contribution ) , cyclic electron transport plays only a minor role ( below 10 % ) under photoautotrophic conditions for all the strains , while linear electron transport increased up to 5.5-fold from WT to PAL mutant .
	manualset3
98398	4	400205	5	NULL	NULL	0	NULL	 minor role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to mixotrophic conditions ( up to 80 % contribution ) , cyclic electron transport plays only a minor role ( below 10 % ) under photoautotrophic conditions for all the strains , while linear electron transport increased up to 5.5-fold from WT to PAL mutant .
	manualset3
98399	5	400205	5	NULL	NULL	0	NULL	10 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to mixotrophic conditions ( up to 80 % contribution ) , cyclic electron transport plays only a minor role ( below 10 % ) under photoautotrophic conditions for all the strains , while linear electron transport increased up to 5.5-fold from WT to PAL mutant .
	manualset3
98400	6	400205	5	NULL	NULL	0	NULL	photoautotrophic conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to mixotrophic conditions ( up to 80 % contribution ) , cyclic electron transport plays only a minor role ( below 10 % ) under photoautotrophic conditions for all the strains , while linear electron transport increased up to 5.5-fold from WT to PAL mutant .
	manualset3
98401	7	400205	5	NULL	NULL	0	NULL	strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to mixotrophic conditions ( up to 80 % contribution ) , cyclic electron transport plays only a minor role ( below 10 % ) under photoautotrophic conditions for all the strains , while linear electron transport increased up to 5.5-fold from WT to PAL mutant .
	manualset3
98402	8	400205	5	NULL	NULL	0	NULL	linear electron transport	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to mixotrophic conditions ( up to 80 % contribution ) , cyclic electron transport plays only a minor role ( below 10 % ) under photoautotrophic conditions for all the strains , while linear electron transport increased up to 5.5-fold from WT to PAL mutant .
	manualset3
98403	9	400205	5	NULL	NULL	0	NULL	5.5-fold	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to mixotrophic conditions ( up to 80 % contribution ) , cyclic electron transport plays only a minor role ( below 10 % ) under photoautotrophic conditions for all the strains , while linear electron transport increased up to 5.5-fold from WT to PAL mutant .
	manualset3
98404	10	400205	5	NULL	NULL	0	NULL	WT	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to mixotrophic conditions ( up to 80 % contribution ) , cyclic electron transport plays only a minor role ( below 10 % ) under photoautotrophic conditions for all the strains , while linear electron transport increased up to 5.5-fold from WT to PAL mutant .
	manualset3
98405	11	400205	5	NULL	NULL	0	NULL	PAL mutant	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to mixotrophic conditions ( up to 80 % contribution ) , cyclic electron transport plays only a minor role ( below 10 % ) under photoautotrophic conditions for all the strains , while linear electron transport increased up to 5.5-fold from WT to PAL mutant .
	manualset3
98406	1	400206	5	NULL	NULL	0	NULL	Wunderlich syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Wunderlich syndrome : presentation of a case ) .
	manualset3
98407	2	400206	5	NULL	NULL	0	NULL	presentation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Wunderlich syndrome : presentation of a case ) .
	manualset3
98408	3	400206	5	NULL	NULL	0	NULL	case	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( Wunderlich syndrome : presentation of a case ) .
	manualset3
98409	1	400207	5	NULL	NULL	NULL	NULL	nursing homes	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast to nursing homes , AL allows residents to experience continuities with self and home : a private room , some of their own belongings , and access to relationships and activities associated with self and home .
	manualset3
98410	2	400207	5	NULL	NULL	0	NULL	AL	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to nursing homes , AL allows residents to experience continuities with self and home : a private room , some of their own belongings , and access to relationships and activities associated with self and home .
	manualset3
98411	3	400207	5	NULL	NULL	0	NULL	residents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to nursing homes , AL allows residents to experience continuities with self and home : a private room , some of their own belongings , and access to relationships and activities associated with self and home .
	manualset3
98412	4	400207	5	NULL	NULL	0	NULL	self 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to nursing homes , AL allows residents to experience continuities with self and home : a private room , some of their own belongings , and access to relationships and activities associated with self and home .
	manualset3
98413	5	400207	5	NULL	NULL	0	NULL	home	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to nursing homes , AL allows residents to experience continuities with self and home : a private room , some of their own belongings , and access to relationships and activities associated with self and home .
	manualset3
98414	6	400207	5	NULL	NULL	0	NULL	a private room	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to nursing homes , AL allows residents to experience continuities with self and home : a private room , some of their own belongings , and access to relationships and activities associated with self and home .
	manualset3
98415	7	400207	5	NULL	NULL	0	NULL	own belongings	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to nursing homes , AL allows residents to experience continuities with self and home : a private room , some of their own belongings , and access to relationships and activities associated with self and home .
	manualset3
98416	8	400207	5	NULL	NULL	0	NULL	relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to nursing homes , AL allows residents to experience continuities with self and home : a private room , some of their own belongings , and access to relationships and activities associated with self and home .
	manualset3
98417	9	400207	5	NULL	NULL	0	NULL	activities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to nursing homes , AL allows residents to experience continuities with self and home : a private room , some of their own belongings , and access to relationships and activities associated with self and home .
	manualset3
98418	10	400207	5	NULL	NULL	0	NULL	self	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to nursing homes , AL allows residents to experience continuities with self and home : a private room , some of their own belongings , and access to relationships and activities associated with self and home .
	manualset3
98419	11	400207	5	NULL	NULL	0	NULL	home	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to nursing homes , AL allows residents to experience continuities with self and home : a private room , some of their own belongings , and access to relationships and activities associated with self and home .
	manualset3
98420	1	400208	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to patients with senile dementia , in these HD patients glucose utilization typically was normal throughout the rest of the brain , regardless of the severity of symptoms and despite apparent shrinkage of brain tissue .
	manualset3
98421	2	400208	5	NULL	NULL	0	NULL	senile dementia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to patients with senile dementia , in these HD patients glucose utilization typically was normal throughout the rest of the brain , regardless of the severity of symptoms and despite apparent shrinkage of brain tissue .
	manualset3
98422	3	400208	5	NULL	NULL	0	NULL	HD patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to patients with senile dementia , in these HD patients glucose utilization typically was normal throughout the rest of the brain , regardless of the severity of symptoms and despite apparent shrinkage of brain tissue .
	manualset3
98423	4	400208	5	NULL	NULL	0	NULL	glucose utilization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to patients with senile dementia , in these HD patients glucose utilization typically was normal throughout the rest of the brain , regardless of the severity of symptoms and despite apparent shrinkage of brain tissue .
	manualset3
98424	5	400208	5	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to patients with senile dementia , in these HD patients glucose utilization typically was normal throughout the rest of the brain , regardless of the severity of symptoms and despite apparent shrinkage of brain tissue .
	manualset3
98425	6	400208	5	NULL	NULL	0	NULL	severity of symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to patients with senile dementia , in these HD patients glucose utilization typically was normal throughout the rest of the brain , regardless of the severity of symptoms and despite apparent shrinkage of brain tissue .
	manualset3
98426	7	400208	5	NULL	NULL	0	NULL	apparent shrinkage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to patients with senile dementia , in these HD patients glucose utilization typically was normal throughout the rest of the brain , regardless of the severity of symptoms and despite apparent shrinkage of brain tissue .
	manualset3
98427	8	400208	5	NULL	NULL	0	NULL	brain tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to patients with senile dementia , in these HD patients glucose utilization typically was normal throughout the rest of the brain , regardless of the severity of symptoms and despite apparent shrinkage of brain tissue .
	manualset3
98428	1	400209	5	NULL	NULL	0	NULL	WT therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the WT therapy , which must preserve the electrotemporal code , the VT therapy can operate also with postsynaptic agonists .
	manualset3
98429	2	400209	5	NULL	NULL	NULL	NULL	electrotemporal code	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast to the WT therapy , which must preserve the electrotemporal code , the VT therapy can operate also with postsynaptic agonists .
	manualset3
98430	3	400209	5	NULL	NULL	0	NULL	VT therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the WT therapy , which must preserve the electrotemporal code , the VT therapy can operate also with postsynaptic agonists .
	manualset3
98431	4	400209	5	NULL	NULL	0	NULL	postsynaptic agonists	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the WT therapy , which must preserve the electrotemporal code , the VT therapy can operate also with postsynaptic agonists .
	manualset3
98432	1	400210	5	NULL	NULL	0	NULL	atrazine adsorption behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the atrazine adsorption behavior of powdered activated carbon ( PAC ) , LAM showed a persistent adsorption capacity for atrazine when initial concentrations of 0.57 , 1.12 , 8.31 and 19.01 mg/L were present , and the equilibrium time was 12 hr .
	manualset3
98433	2	400210	5	NULL	NULL	0	NULL	powdered activated carbon ( PAC )	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the atrazine adsorption behavior of powdered activated carbon ( PAC ) , LAM showed a persistent adsorption capacity for atrazine when initial concentrations of 0.57 , 1.12 , 8.31 and 19.01 mg/L were present , and the equilibrium time was 12 hr .
	manualset3
98434	3	400210	5	NULL	NULL	0	NULL	LAM	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the atrazine adsorption behavior of powdered activated carbon ( PAC ) , LAM showed a persistent adsorption capacity for atrazine when initial concentrations of 0.57 , 1.12 , 8.31 and 19.01 mg/L were present , and the equilibrium time was 12 hr .
	manualset3
98435	4	400210	5	NULL	NULL	0	NULL	persistent adsorption capacity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the atrazine adsorption behavior of powdered activated carbon ( PAC ) , LAM showed a persistent adsorption capacity for atrazine when initial concentrations of 0.57 , 1.12 , 8.31 and 19.01 mg/L were present , and the equilibrium time was 12 hr .
	manualset3
98436	5	400210	5	NULL	NULL	0	NULL	atrazine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the atrazine adsorption behavior of powdered activated carbon ( PAC ) , LAM showed a persistent adsorption capacity for atrazine when initial concentrations of 0.57 , 1.12 , 8.31 and 19.01 mg/L were present , and the equilibrium time was 12 hr .
	manualset3
98437	6	400210	5	NULL	NULL	0	NULL	initial concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the atrazine adsorption behavior of powdered activated carbon ( PAC ) , LAM showed a persistent adsorption capacity for atrazine when initial concentrations of 0.57 , 1.12 , 8.31 and 19.01 mg/L were present , and the equilibrium time was 12 hr .
	manualset3
98438	7	400210	5	NULL	NULL	0	NULL	0.57 , 1.12 , 8.31 and 19.01 mg/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the atrazine adsorption behavior of powdered activated carbon ( PAC ) , LAM showed a persistent adsorption capacity for atrazine when initial concentrations of 0.57 , 1.12 , 8.31 and 19.01 mg/L were present , and the equilibrium time was 12 hr .
	manualset3
98439	8	400210	5	NULL	NULL	0	NULL	equilibrium time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the atrazine adsorption behavior of powdered activated carbon ( PAC ) , LAM showed a persistent adsorption capacity for atrazine when initial concentrations of 0.57 , 1.12 , 8.31 and 19.01 mg/L were present , and the equilibrium time was 12 hr .
	manualset3
98440	9	400210	5	NULL	NULL	0	NULL	12 hr	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the atrazine adsorption behavior of powdered activated carbon ( PAC ) , LAM showed a persistent adsorption capacity for atrazine when initial concentrations of 0.57 , 1.12 , 8.31 and 19.01 mg/L were present , and the equilibrium time was 12 hr .
	manualset3
98441	1	400211	5	NULL	NULL	0	NULL	cancer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the cancer cells , the normal lung fibroblasts ( CCL-151 ) did not show any increase in ROS and were resistant to CLEFMA-induced cell death .
	manualset3
98442	2	400211	5	NULL	NULL	0	NULL	normal lung fibroblasts ( CCL-151 )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the cancer cells , the normal lung fibroblasts ( CCL-151 ) did not show any increase in ROS and were resistant to CLEFMA-induced cell death .
	manualset3
98443	3	400211	5	NULL	NULL	0	NULL	ROS	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the cancer cells , the normal lung fibroblasts ( CCL-151 ) did not show any increase in ROS and were resistant to CLEFMA-induced cell death .
	manualset3
98444	4	400211	5	NULL	NULL	NULL	NULL	CLEFMA-induced cell death	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast to the cancer cells , the normal lung fibroblasts ( CCL-151 ) did not show any increase in ROS and were resistant to CLEFMA-induced cell death .
	manualset3
98445	2	400212	5	NULL	NULL	NULL	NULL	non-immunized rats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast to the findings in non-immunized rats , the rejection process in pre-immunized rats was characterized by marked intragraft infiltration by macrophages 3 days after transplantation .
	manualset3
98446	1	400212	5	NULL	NULL	0	NULL	finding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the findings in non-immunized rats , the rejection process in pre-immunized rats was characterized by marked intragraft infiltration by macrophages 3 days after transplantation .
	manualset3
98447	3	400212	5	NULL	NULL	NULL	NULL	 rejection process	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast to the findings in non-immunized rats , the rejection process in pre-immunized rats was characterized by marked intragraft infiltration by macrophages 3 days after transplantation .
	manualset3
98448	4	400212	5	NULL	NULL	0	NULL	pre-immunized rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the findings in non-immunized rats , the rejection process in pre-immunized rats was characterized by marked intragraft infiltration by macrophages 3 days after transplantation .
	manualset3
98449	5	400212	5	NULL	NULL	NULL	NULL	intragraft infiltration	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast to the findings in non-immunized rats , the rejection process in pre-immunized rats was characterized by marked intragraft infiltration by macrophages 3 days after transplantation .
	manualset3
98450	6	400212	5	NULL	NULL	0	NULL	macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the findings in non-immunized rats , the rejection process in pre-immunized rats was characterized by marked intragraft infiltration by macrophages 3 days after transplantation .
	manualset3
98451	7	400212	5	NULL	NULL	0	NULL	3 days	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the findings in non-immunized rats , the rejection process in pre-immunized rats was characterized by marked intragraft infiltration by macrophages 3 days after transplantation .
	manualset3
98452	8	400212	5	NULL	NULL	0	NULL	transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the findings in non-immunized rats , the rejection process in pre-immunized rats was characterized by marked intragraft infiltration by macrophages 3 days after transplantation .
	manualset3
98453	1	400213	5	NULL	NULL	0	NULL	triblock `` PEG/PPG/PEG '' sample designation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the indicated triblock `` PEG/PPG/PEG '' sample designation of this commercial surfactant , all of these oligomers are found to consist primarily of diblock PEG/PPG structures , so that their termini differ significantly in hydrophobicity , as expected for a surfactant .
	manualset3
98454	2	400213	5	NULL	NULL	NULL	NULL	commercial surfactant 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast to the indicated triblock `` PEG/PPG/PEG '' sample designation of this commercial surfactant , all of these oligomers are found to consist primarily of diblock PEG/PPG structures , so that their termini differ significantly in hydrophobicity , as expected for a surfactant .
	manualset3
98455	3	400213	5	NULL	NULL	NULL	NULL	oligomers	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast to the indicated triblock `` PEG/PPG/PEG '' sample designation of this commercial surfactant , all of these oligomers are found to consist primarily of diblock PEG/PPG structures , so that their termini differ significantly in hydrophobicity , as expected for a surfactant .
	manualset3
98456	4	400213	5	NULL	NULL	NULL	NULL	diblock PEG/PPG structures	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast to the indicated triblock `` PEG/PPG/PEG '' sample designation of this commercial surfactant , all of these oligomers are found to consist primarily of diblock PEG/PPG structures , so that their termini differ significantly in hydrophobicity , as expected for a surfactant .
	manualset3
98457	5	400213	5	NULL	NULL	0	NULL	termini	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the indicated triblock `` PEG/PPG/PEG '' sample designation of this commercial surfactant , all of these oligomers are found to consist primarily of diblock PEG/PPG structures , so that their termini differ significantly in hydrophobicity , as expected for a surfactant .
	manualset3
98458	6	400213	5	NULL	NULL	0	NULL	hydrophobicity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the indicated triblock `` PEG/PPG/PEG '' sample designation of this commercial surfactant , all of these oligomers are found to consist primarily of diblock PEG/PPG structures , so that their termini differ significantly in hydrophobicity , as expected for a surfactant .
	manualset3
98459	7	400213	5	NULL	NULL	0	NULL	surfactant 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the indicated triblock `` PEG/PPG/PEG '' sample designation of this commercial surfactant , all of these oligomers are found to consist primarily of diblock PEG/PPG structures , so that their termini differ significantly in hydrophobicity , as expected for a surfactant .
	manualset3
98460	1	400214	5	NULL	NULL	0	NULL	malignant cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the malignant cells , normal mammary epithelial cells did not adsorb erythrocytes coated with as much as 100 microgram Con A per ml .
	manualset3
98461	2	400214	5	NULL	NULL	0	NULL	normal mammary epithelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the malignant cells , normal mammary epithelial cells did not adsorb erythrocytes coated with as much as 100 microgram Con A per ml .
	manualset3
98462	3	400214	5	NULL	NULL	0	NULL	erythrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the malignant cells , normal mammary epithelial cells did not adsorb erythrocytes coated with as much as 100 microgram Con A per ml .
	manualset3
98463	4	400214	5	NULL	NULL	0	NULL	100 microgram Con A per ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the malignant cells , normal mammary epithelial cells did not adsorb erythrocytes coated with as much as 100 microgram Con A per ml .
	manualset3
98464	1	400215	5	NULL	NULL	0	NULL	streptococci of groups A , C and G	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the streptococci of groups A , C and G , the group-B streptococci interacted more with the alpha , beta-chain of fibrinogen than with whole fibrinogen .
	manualset3
98465	2	400215	5	NULL	NULL	0	NULL	group-B streptococci	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the streptococci of groups A , C and G , the group-B streptococci interacted more with the alpha , beta-chain of fibrinogen than with whole fibrinogen .
	manualset3
98466	3	400215	5	NULL	NULL	NULL	NULL	alpha , beta-chain of fibrinogen	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast to the streptococci of groups A , C and G , the group-B streptococci interacted more with the alpha , beta-chain of fibrinogen than with whole fibrinogen .
	manualset3
98467	4	400215	5	NULL	NULL	0	NULL	whole fibrinogen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the streptococci of groups A , C and G , the group-B streptococci interacted more with the alpha , beta-chain of fibrinogen than with whole fibrinogen .
	manualset3
98468	1	400216	5	NULL	NULL	0	NULL	ubiquitous expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the ubiquitous expression of mu - and m-types , Northern blot analysis revealed that the mRNA for p94 exists only in skeletal muscle with none detected in other tissues including heart muscle and smooth muscles such as intestine .
	manualset3
98469	2	400216	5	NULL	NULL	0	NULL	mu -type	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the ubiquitous expression of mu - and m-types , Northern blot analysis revealed that the mRNA for p94 exists only in skeletal muscle with none detected in other tissues including heart muscle and smooth muscles such as intestine .
	manualset3
98470	3	400216	5	NULL	NULL	0	NULL	m-type	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the ubiquitous expression of mu - and m-types , Northern blot analysis revealed that the mRNA for p94 exists only in skeletal muscle with none detected in other tissues including heart muscle and smooth muscles such as intestine .
	manualset3
98471	4	400216	5	NULL	NULL	0	NULL	Northern blot analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the ubiquitous expression of mu - and m-types , Northern blot analysis revealed that the mRNA for p94 exists only in skeletal muscle with none detected in other tissues including heart muscle and smooth muscles such as intestine .
	manualset3
98472	5	400216	5	NULL	NULL	0	NULL	mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the ubiquitous expression of mu - and m-types , Northern blot analysis revealed that the mRNA for p94 exists only in skeletal muscle with none detected in other tissues including heart muscle and smooth muscles such as intestine .
	manualset3
98473	6	400216	5	NULL	NULL	0	NULL	p94	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the ubiquitous expression of mu - and m-types , Northern blot analysis revealed that the mRNA for p94 exists only in skeletal muscle with none detected in other tissues including heart muscle and smooth muscles such as intestine .
	manualset3
98474	7	400216	5	NULL	NULL	0	NULL	skeletal muscle	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the ubiquitous expression of mu - and m-types , Northern blot analysis revealed that the mRNA for p94 exists only in skeletal muscle with none detected in other tissues including heart muscle and smooth muscles such as intestine .
	manualset3
98475	8	400216	5	NULL	NULL	0	NULL	tissues 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the ubiquitous expression of mu - and m-types , Northern blot analysis revealed that the mRNA for p94 exists only in skeletal muscle with none detected in other tissues including heart muscle and smooth muscles such as intestine .
	manualset3
98476	9	400216	5	NULL	NULL	0	NULL	heart muscle	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the ubiquitous expression of mu - and m-types , Northern blot analysis revealed that the mRNA for p94 exists only in skeletal muscle with none detected in other tissues including heart muscle and smooth muscles such as intestine .
	manualset3
98477	10	400216	5	NULL	NULL	0	NULL	smooth muscles	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the ubiquitous expression of mu - and m-types , Northern blot analysis revealed that the mRNA for p94 exists only in skeletal muscle with none detected in other tissues including heart muscle and smooth muscles such as intestine .
	manualset3
98478	11	400216	5	NULL	NULL	0	NULL	intestine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the ubiquitous expression of mu - and m-types , Northern blot analysis revealed that the mRNA for p94 exists only in skeletal muscle with none detected in other tissues including heart muscle and smooth muscles such as intestine .
	manualset3
98479	1	400217	5	NULL	NULL	0	NULL	Southern Europe	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to this , in Southern Europe and in Arab countries zoophilic dermatophytes , such as M. canis and T. verrucosum , are the most frequently isolated dermatophytes .
	manualset3
98480	2	400217	5	NULL	NULL	0	NULL	Arab countries	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to this , in Southern Europe and in Arab countries zoophilic dermatophytes , such as M. canis and T. verrucosum , are the most frequently isolated dermatophytes .
	manualset3
98481	3	400217	5	NULL	NULL	0	NULL	zoophilic dermatophytes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to this , in Southern Europe and in Arab countries zoophilic dermatophytes , such as M. canis and T. verrucosum , are the most frequently isolated dermatophytes .
	manualset3
98482	4	400217	5	NULL	NULL	0	NULL	M. canis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to this , in Southern Europe and in Arab countries zoophilic dermatophytes , such as M. canis and T. verrucosum , are the most frequently isolated dermatophytes .
	manualset3
98483	5	400217	5	NULL	NULL	0	NULL	T. verrucosum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to this , in Southern Europe and in Arab countries zoophilic dermatophytes , such as M. canis and T. verrucosum , are the most frequently isolated dermatophytes .
	manualset3
98484	6	400217	5	NULL	NULL	0	NULL	dermatophytes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to this , in Southern Europe and in Arab countries zoophilic dermatophytes , such as M. canis and T. verrucosum , are the most frequently isolated dermatophytes .
	manualset3
98485	1	400218	5	NULL	NULL	0	NULL	white matter lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to white matter lesions , cortical multiple sclerosis lesions are accompanied by only minor inflammation .
	manualset3
98486	2	400218	5	NULL	NULL	0	NULL	cortical multiple sclerosis lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to white matter lesions , cortical multiple sclerosis lesions are accompanied by only minor inflammation .
	manualset3
98487	3	400218	5	NULL	NULL	0	NULL	minor inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to white matter lesions , cortical multiple sclerosis lesions are accompanied by only minor inflammation .
	manualset3
98488	1	400219	5	NULL	NULL	0	NULL	wide-spread belief	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to wide-spread belief , metabolic control is only marginally better in summer compared to winter .
	manualset3
98489	2	400219	5	NULL	NULL	0	NULL	metabolic control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to wide-spread belief , metabolic control is only marginally better in summer compared to winter .
	manualset3
98490	3	400219	5	NULL	NULL	0	NULL	summer	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to wide-spread belief , metabolic control is only marginally better in summer compared to winter .
	manualset3
98491	4	400219	5	NULL	NULL	0	NULL	winter	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to wide-spread belief , metabolic control is only marginally better in summer compared to winter .
	manualset3
98492	1	400220	5	NULL	NULL	0	NULL	control	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In control and sterile inflammation , functional hepatectomy was associated with significant decreases ( P less than .05 ) in BCAA .
	manualset3
98493	2	400220	5	NULL	NULL	0	NULL	sterile inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In control and sterile inflammation , functional hepatectomy was associated with significant decreases ( P less than .05 ) in BCAA .
	manualset3
98494	3	400220	5	NULL	NULL	0	NULL	functional hepatectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In control and sterile inflammation , functional hepatectomy was associated with significant decreases ( P less than .05 ) in BCAA .
	manualset3
98495	4	400220	5	NULL	NULL	0	NULL	P less than .05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In control and sterile inflammation , functional hepatectomy was associated with significant decreases ( P less than .05 ) in BCAA .
	manualset3
98496	5	400220	5	NULL	NULL	0	NULL	BCAA	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In control and sterile inflammation , functional hepatectomy was associated with significant decreases ( P less than .05 ) in BCAA .
	manualset3
98497	1	400221	5	NULL	NULL	0	NULL	control rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In control rats , EC-SOD mRNA was synthesized in macrophages and in cells of the arterial vessel walls and the alveolar septa .
	manualset3
98498	2	400221	5	NULL	NULL	0	NULL	EC-SOD mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In control rats , EC-SOD mRNA was synthesized in macrophages and in cells of the arterial vessel walls and the alveolar septa .
	manualset3
98499	3	400221	5	NULL	NULL	0	NULL	macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In control rats , EC-SOD mRNA was synthesized in macrophages and in cells of the arterial vessel walls and the alveolar septa .
	manualset3
98500	4	400221	5	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In control rats , EC-SOD mRNA was synthesized in macrophages and in cells of the arterial vessel walls and the alveolar septa .
	manualset3
98501	5	400221	5	NULL	NULL	0	NULL	arterial vessel walls	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In control rats , EC-SOD mRNA was synthesized in macrophages and in cells of the arterial vessel walls and the alveolar septa .
	manualset3
98502	6	400221	5	NULL	NULL	0	NULL	alveolar septa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In control rats , EC-SOD mRNA was synthesized in macrophages and in cells of the arterial vessel walls and the alveolar septa .
	manualset3
98503	1	400222	5	NULL	NULL	0	NULL	conventional agarose electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conventional agarose electrophoresis , voltage gradient was found to be the determining parameter in the separation of SC DNA .
	manualset3
98504	2	400222	5	NULL	NULL	0	NULL	voltage gradient	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conventional agarose electrophoresis , voltage gradient was found to be the determining parameter in the separation of SC DNA .
	manualset3
98505	3	400222	5	NULL	NULL	0	NULL	parameter	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In conventional agarose electrophoresis , voltage gradient was found to be the determining parameter in the separation of SC DNA .
	manualset3
98506	4	400222	5	NULL	NULL	0	NULL	separation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conventional agarose electrophoresis , voltage gradient was found to be the determining parameter in the separation of SC DNA .
	manualset3
98507	5	400222	5	NULL	NULL	0	NULL	SC DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In conventional agarose electrophoresis , voltage gradient was found to be the determining parameter in the separation of SC DNA .
	manualset3
98508	1	400223	5	NULL	NULL	0	NULL	cultured cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In cultured cells , the OSR1 ( rs12329305 ) ( T ) allele produced no identifiable transcript .
	manualset3
98509	2	400223	5	NULL	NULL	0	NULL	OSR1 ( rs12329305 ) ( T ) allele	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In cultured cells , the OSR1 ( rs12329305 ) ( T ) allele produced no identifiable transcript .
	manualset3
98510	3	400223	5	NULL	NULL	0	NULL	transcript 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In cultured cells , the OSR1 ( rs12329305 ) ( T ) allele produced no identifiable transcript .
	manualset3
98511	1	400224	5	NULL	NULL	0	NULL	cultures 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In cultures at more mature stages ( 14 days in culture ) bromide treatment did not lead to formation of low affinity GABA receptors .
	manualset3
98512	2	400224	5	NULL	NULL	0	NULL	mature stages	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In cultures at more mature stages ( 14 days in culture ) bromide treatment did not lead to formation of low affinity GABA receptors .
	manualset3
98513	3	400224	5	NULL	NULL	0	NULL	14 days	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In cultures at more mature stages ( 14 days in culture ) bromide treatment did not lead to formation of low affinity GABA receptors .
	manualset3
98514	4	400224	5	NULL	NULL	0	NULL	culture 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In cultures at more mature stages ( 14 days in culture ) bromide treatment did not lead to formation of low affinity GABA receptors .
	manualset3
98515	5	400224	5	NULL	NULL	0	NULL	bromide treatment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In cultures at more mature stages ( 14 days in culture ) bromide treatment did not lead to formation of low affinity GABA receptors .
	manualset3
98516	6	400224	5	NULL	NULL	0	NULL	formation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In cultures at more mature stages ( 14 days in culture ) bromide treatment did not lead to formation of low affinity GABA receptors .
	manualset3
98517	7	400224	5	NULL	NULL	0	NULL	low affinity GABA receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In cultures at more mature stages ( 14 days in culture ) bromide treatment did not lead to formation of low affinity GABA receptors .
	manualset3
98518	1	400225	5	NULL	NULL	0	NULL	discrepancy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In despite of the discrepancy in the warming effect among different regions and seasons , this energy-saving facility was reliable for the field research on crop responses to climate warming , when the homogeneity of increased temperature , the effective area , and the effects on crop growth period were taken into comprehensive consideration .
	manualset3
98519	2	400225	5	NULL	NULL	0	NULL	warming effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In despite of the discrepancy in the warming effect among different regions and seasons , this energy-saving facility was reliable for the field research on crop responses to climate warming , when the homogeneity of increased temperature , the effective area , and the effects on crop growth period were taken into comprehensive consideration .
	manualset3
98520	3	400225	5	NULL	NULL	0	NULL	different regions	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In despite of the discrepancy in the warming effect among different regions and seasons , this energy-saving facility was reliable for the field research on crop responses to climate warming , when the homogeneity of increased temperature , the effective area , and the effects on crop growth period were taken into comprehensive consideration .
	manualset3
98521	4	400225	5	NULL	NULL	0	NULL	seasons	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In despite of the discrepancy in the warming effect among different regions and seasons , this energy-saving facility was reliable for the field research on crop responses to climate warming , when the homogeneity of increased temperature , the effective area , and the effects on crop growth period were taken into comprehensive consideration .
	manualset3
98522	5	400225	5	NULL	NULL	0	NULL	energy-saving facility	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In despite of the discrepancy in the warming effect among different regions and seasons , this energy-saving facility was reliable for the field research on crop responses to climate warming , when the homogeneity of increased temperature , the effective area , and the effects on crop growth period were taken into comprehensive consideration .
	manualset3
98523	6	400225	5	NULL	NULL	0	NULL	field research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In despite of the discrepancy in the warming effect among different regions and seasons , this energy-saving facility was reliable for the field research on crop responses to climate warming , when the homogeneity of increased temperature , the effective area , and the effects on crop growth period were taken into comprehensive consideration .
	manualset3
98524	7	400225	5	NULL	NULL	0	NULL	crop responses	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In despite of the discrepancy in the warming effect among different regions and seasons , this energy-saving facility was reliable for the field research on crop responses to climate warming , when the homogeneity of increased temperature , the effective area , and the effects on crop growth period were taken into comprehensive consideration .
	manualset3
98525	8	400225	5	NULL	NULL	0	NULL	climate warming 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In despite of the discrepancy in the warming effect among different regions and seasons , this energy-saving facility was reliable for the field research on crop responses to climate warming , when the homogeneity of increased temperature , the effective area , and the effects on crop growth period were taken into comprehensive consideration .
	manualset3
98526	9	400225	5	NULL	NULL	0	NULL	homogeneity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In despite of the discrepancy in the warming effect among different regions and seasons , this energy-saving facility was reliable for the field research on crop responses to climate warming , when the homogeneity of increased temperature , the effective area , and the effects on crop growth period were taken into comprehensive consideration .
	manualset3
98527	10	400225	5	NULL	NULL	0	NULL	increased temperature 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In despite of the discrepancy in the warming effect among different regions and seasons , this energy-saving facility was reliable for the field research on crop responses to climate warming , when the homogeneity of increased temperature , the effective area , and the effects on crop growth period were taken into comprehensive consideration .
	manualset3
98528	11	400225	5	NULL	NULL	0	NULL	effective area	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In despite of the discrepancy in the warming effect among different regions and seasons , this energy-saving facility was reliable for the field research on crop responses to climate warming , when the homogeneity of increased temperature , the effective area , and the effects on crop growth period were taken into comprehensive consideration .
	manualset3
98529	12	400225	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In despite of the discrepancy in the warming effect among different regions and seasons , this energy-saving facility was reliable for the field research on crop responses to climate warming , when the homogeneity of increased temperature , the effective area , and the effects on crop growth period were taken into comprehensive consideration .
	manualset3
98530	13	400225	5	NULL	NULL	0	NULL	crop growth period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In despite of the discrepancy in the warming effect among different regions and seasons , this energy-saving facility was reliable for the field research on crop responses to climate warming , when the homogeneity of increased temperature , the effective area , and the effects on crop growth period were taken into comprehensive consideration .
	manualset3
98531	14	400225	5	NULL	NULL	0	NULL	comprehensive consideration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In despite of the discrepancy in the warming effect among different regions and seasons , this energy-saving facility was reliable for the field research on crop responses to climate warming , when the homogeneity of increased temperature , the effective area , and the effects on crop growth period were taken into comprehensive consideration .
	manualset3
98532	1	400226	5	NULL	NULL	0	NULL	diabetic rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In diabetic rats , except for UDP-GAL , all pools were increased 41 to 68 % .
	manualset3
98533	2	400226	5	NULL	NULL	0	NULL	UDP-GAL	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In diabetic rats , except for UDP-GAL , all pools were increased 41 to 68 % .
	manualset3
98534	3	400226	5	NULL	NULL	0	NULL	pools	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In diabetic rats , except for UDP-GAL , all pools were increased 41 to 68 % .
	manualset3
98535	4	400226	5	NULL	NULL	0	NULL	41 to 68 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In diabetic rats , except for UDP-GAL , all pools were increased 41 to 68 % .
	manualset3
98536	1	400227	5	NULL	NULL	0	NULL	different scenarios	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In different scenarios of constant , increasing , or decreasing caries-controlling effects , and of limited ( age 6-18 yr ) or lifelong application , the combination of fluoride salt , fluoride toothpaste , and fluoride gel were most cost-effective .
	manualset3
98537	2	400227	5	NULL	NULL	0	NULL	controlling effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In different scenarios of constant , increasing , or decreasing caries-controlling effects , and of limited ( age 6-18 yr ) or lifelong application , the combination of fluoride salt , fluoride toothpaste , and fluoride gel were most cost-effective .
	manualset3
98538	3	400227	5	NULL	NULL	0	NULL	 limited application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In different scenarios of constant , increasing , or decreasing caries-controlling effects , and of limited ( age 6-18 yr ) or lifelong application , the combination of fluoride salt , fluoride toothpaste , and fluoride gel were most cost-effective .
	manualset3
98539	4	400227	5	NULL	NULL	0	NULL	age	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In different scenarios of constant , increasing , or decreasing caries-controlling effects , and of limited ( age 6-18 yr ) or lifelong application , the combination of fluoride salt , fluoride toothpaste , and fluoride gel were most cost-effective .
	manualset3
98540	5	400227	5	NULL	NULL	0	NULL	6-18 yr	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In different scenarios of constant , increasing , or decreasing caries-controlling effects , and of limited ( age 6-18 yr ) or lifelong application , the combination of fluoride salt , fluoride toothpaste , and fluoride gel were most cost-effective .
	manualset3
98541	6	400227	5	NULL	NULL	0	NULL	lifelong application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In different scenarios of constant , increasing , or decreasing caries-controlling effects , and of limited ( age 6-18 yr ) or lifelong application , the combination of fluoride salt , fluoride toothpaste , and fluoride gel were most cost-effective .
	manualset3
98542	7	400227	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In different scenarios of constant , increasing , or decreasing caries-controlling effects , and of limited ( age 6-18 yr ) or lifelong application , the combination of fluoride salt , fluoride toothpaste , and fluoride gel were most cost-effective .
	manualset3
98543	8	400227	5	NULL	NULL	0	NULL	fluoride salt	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In different scenarios of constant , increasing , or decreasing caries-controlling effects , and of limited ( age 6-18 yr ) or lifelong application , the combination of fluoride salt , fluoride toothpaste , and fluoride gel were most cost-effective .
	manualset3
98544	9	400227	5	NULL	NULL	0	NULL	fluoride toothpaste	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In different scenarios of constant , increasing , or decreasing caries-controlling effects , and of limited ( age 6-18 yr ) or lifelong application , the combination of fluoride salt , fluoride toothpaste , and fluoride gel were most cost-effective .
	manualset3
98545	10	400227	5	NULL	NULL	0	NULL	fluoride gel 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In different scenarios of constant , increasing , or decreasing caries-controlling effects , and of limited ( age 6-18 yr ) or lifelong application , the combination of fluoride salt , fluoride toothpaste , and fluoride gel were most cost-effective .
	manualset3
98546	1	400228	5	NULL	NULL	0	NULL	 diffuse large B-cell NHL	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In diffuse large B-cell NHL , Bcl-2 , Bcl-X , and Bax expression alone or in combination is associated with chemoresistance and shortterm survival .
	manualset3
98547	2	400228	5	NULL	NULL	0	NULL	Bcl-2 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In diffuse large B-cell NHL , Bcl-2 , Bcl-X , and Bax expression alone or in combination is associated with chemoresistance and shortterm survival .
	manualset3
98548	3	400228	5	NULL	NULL	0	NULL	Bcl-X expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In diffuse large B-cell NHL , Bcl-2 , Bcl-X , and Bax expression alone or in combination is associated with chemoresistance and shortterm survival .
	manualset3
98549	4	400228	5	NULL	NULL	0	NULL	Bax expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In diffuse large B-cell NHL , Bcl-2 , Bcl-X , and Bax expression alone or in combination is associated with chemoresistance and shortterm survival .
	manualset3
98550	5	400228	5	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In diffuse large B-cell NHL , Bcl-2 , Bcl-X , and Bax expression alone or in combination is associated with chemoresistance and shortterm survival .
	manualset3
98551	6	400228	5	NULL	NULL	NULL	NULL	chemoresistance	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In diffuse large B-cell NHL , Bcl-2 , Bcl-X , and Bax expression alone or in combination is associated with chemoresistance and shortterm survival .
	manualset3
98552	7	400228	5	NULL	NULL	0	NULL	shortterm survival	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In diffuse large B-cell NHL , Bcl-2 , Bcl-X , and Bax expression alone or in combination is associated with chemoresistance and shortterm survival .
	manualset3
98553	1	400229	5	NULL	NULL	0	NULL	pilot rehabilitation clinic	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( 2 ) At the pilot rehabilitation clinic a counselling service for patients under a case management trial scheme was established .
	manualset3
98554	2	400229	5	NULL	NULL	0	NULL	counselling service	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( 2 ) At the pilot rehabilitation clinic a counselling service for patients under a case management trial scheme was established .
	manualset3
98555	3	400229	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( 2 ) At the pilot rehabilitation clinic a counselling service for patients under a case management trial scheme was established .
	manualset3
98556	4	400229	5	NULL	NULL	0	NULL	case management trial scheme	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( 2 ) At the pilot rehabilitation clinic a counselling service for patients under a case management trial scheme was established .
	manualset3
98557	1	400230	5	NULL	NULL	0	NULL	Antineoplastic action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Antineoplastic action and toxicity of probimane and its effect on immunologic functions in mice ) .
	manualset3
98558	2	400230	5	NULL	NULL	0	NULL	toxicity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Antineoplastic action and toxicity of probimane and its effect on immunologic functions in mice ) .
	manualset3
98559	3	400230	5	NULL	NULL	0	NULL	probimane 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Antineoplastic action and toxicity of probimane and its effect on immunologic functions in mice ) .
	manualset3
98560	4	400230	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Antineoplastic action and toxicity of probimane and its effect on immunologic functions in mice ) .
	manualset3
98561	5	400230	5	NULL	NULL	0	NULL	immunologic functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Antineoplastic action and toxicity of probimane and its effect on immunologic functions in mice ) .
	manualset3
98562	6	400230	5	NULL	NULL	0	NULL	mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Antineoplastic action and toxicity of probimane and its effect on immunologic functions in mice ) .
	manualset3
98803	1	400231	5	NULL	NULL	0	NULL	risk/benefit report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	( `` The lower , the better : '' this was not confirmed in the risk/benefit report of the ACCORD trial ) .
	manualset3
98804	2	400231	5	NULL	NULL	0	NULL	ACCORD trial	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( `` The lower , the better : '' this was not confirmed in the risk/benefit report of the ACCORD trial ) .
	manualset3
98805	1	400232	5	NULL	NULL	0	NULL	drug discovery	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In drug discovery , LC/MS is relied upon to confirm the identity and assess the purity of chemical entities .
	manualset3
98806	2	400232	5	NULL	NULL	0	NULL	LC/MS	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In drug discovery , LC/MS is relied upon to confirm the identity and assess the purity of chemical entities .
	manualset3
98807	3	400232	5	NULL	NULL	0	NULL	identity	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In drug discovery , LC/MS is relied upon to confirm the identity and assess the purity of chemical entities .
	manualset3
98808	4	400232	5	NULL	NULL	0	NULL	purity	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In drug discovery , LC/MS is relied upon to confirm the identity and assess the purity of chemical entities .
	manualset3
98809	5	400232	5	NULL	NULL	0	NULL	chemical entities	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In drug discovery , LC/MS is relied upon to confirm the identity and assess the purity of chemical entities .
	manualset3
98810	1	400233	5	NULL	NULL	0	NULL	dual infections	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In dual infections of mice with LDV-P and LDV-C all genetic recombinants , like the LDV-C parent itself , had been lost by 7 days p.i. , and only LDV-P persisted .
	manualset3
98811	2	400233	5	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In dual infections of mice with LDV-P and LDV-C all genetic recombinants , like the LDV-C parent itself , had been lost by 7 days p.i. , and only LDV-P persisted .
	manualset3
98812	3	400233	5	NULL	NULL	0	NULL	LDV-P	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In dual infections of mice with LDV-P and LDV-C all genetic recombinants , like the LDV-C parent itself , had been lost by 7 days p.i. , and only LDV-P persisted .
	manualset3
98813	4	400233	5	NULL	NULL	0	NULL	LDV-C	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In dual infections of mice with LDV-P and LDV-C all genetic recombinants , like the LDV-C parent itself , had been lost by 7 days p.i. , and only LDV-P persisted .
	manualset3
98814	5	400233	5	NULL	NULL	0	NULL	genetic recombinants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In dual infections of mice with LDV-P and LDV-C all genetic recombinants , like the LDV-C parent itself , had been lost by 7 days p.i. , and only LDV-P persisted .
	manualset3
100668	6	400233	5	NULL	NULL	0	NULL	 LDV-C parent 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In dual infections of mice with LDV-P and LDV-C all genetic recombinants , like the LDV-C parent itself , had been lost by 7 days p.i. , and only LDV-P persisted .
	manualset3
100669	7	400233	5	NULL	NULL	0	NULL	7 days	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In dual infections of mice with LDV-P and LDV-C all genetic recombinants , like the LDV-C parent itself , had been lost by 7 days p.i. , and only LDV-P persisted .
	manualset3
100670	8	400233	5	NULL	NULL	0	NULL	LDV-P	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In dual infections of mice with LDV-P and LDV-C all genetic recombinants , like the LDV-C parent itself , had been lost by 7 days p.i. , and only LDV-P persisted .
	manualset3
98815	1	400234	5	NULL	NULL	0	NULL	ductus cochlearis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In ductus cochlearis the slope of the linear part of the CM-intensity function was close to unity at most frequencies except the best frequency for the electrode position .
	manualset3
100671	2	400234	5	NULL	NULL	0	NULL	slope of the linear part of the CM-intensity function	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In ductus cochlearis the slope of the linear part of the CM-intensity function was close to unity at most frequencies except the best frequency for the electrode position .
	manualset3
100672	3	400234	5	NULL	NULL	0	NULL	unity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In ductus cochlearis the slope of the linear part of the CM-intensity function was close to unity at most frequencies except the best frequency for the electrode position .
	manualset3
100673	4	400234	5	NULL	NULL	0	NULL	frequencies	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In ductus cochlearis the slope of the linear part of the CM-intensity function was close to unity at most frequencies except the best frequency for the electrode position .
	manualset3
100674	5	400234	5	NULL	NULL	0	NULL	best frequency 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In ductus cochlearis the slope of the linear part of the CM-intensity function was close to unity at most frequencies except the best frequency for the electrode position .
	manualset3
100675	6	400234	5	NULL	NULL	0	NULL	electrode position	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In ductus cochlearis the slope of the linear part of the CM-intensity function was close to unity at most frequencies except the best frequency for the electrode position .
	manualset3
98816	1	400235	5	NULL	NULL	0	NULL	dietary group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In each dietary group , 56 male and 56 female pups were assessed for physical , neuromotor , and reflexologic development postnatally .
	manualset3
98817	2	400235	5	NULL	NULL	0	NULL	 56 male pups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In each dietary group , 56 male and 56 female pups were assessed for physical , neuromotor , and reflexologic development postnatally .
	manualset3
98818	3	400235	5	NULL	NULL	0	NULL	56 female pups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In each dietary group , 56 male and 56 female pups were assessed for physical , neuromotor , and reflexologic development postnatally .
	manualset3
98819	4	400235	5	NULL	NULL	0	NULL	physical development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In each dietary group , 56 male and 56 female pups were assessed for physical , neuromotor , and reflexologic development postnatally .
	manualset3
98820	5	400235	5	NULL	NULL	0	NULL	neuromotor development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In each dietary group , 56 male and 56 female pups were assessed for physical , neuromotor , and reflexologic development postnatally .
	manualset3
98821	6	400235	5	NULL	NULL	0	NULL	reflexologic development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In each dietary group , 56 male and 56 female pups were assessed for physical , neuromotor , and reflexologic development postnatally .
	manualset3
98822	1	400236	5	NULL	NULL	0	NULL	models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In each of these four models , only one input variable ( concentration or bioavailability ) was changed compared with a reference model .
	manualset3
98823	2	400236	5	NULL	NULL	0	NULL	input variable	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In each of these four models , only one input variable ( concentration or bioavailability ) was changed compared with a reference model .
	manualset3
98824	3	400236	5	NULL	NULL	0	NULL	concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In each of these four models , only one input variable ( concentration or bioavailability ) was changed compared with a reference model .
	manualset3
98825	4	400236	5	NULL	NULL	0	NULL	bioavailability	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In each of these four models , only one input variable ( concentration or bioavailability ) was changed compared with a reference model .
	manualset3
98826	5	400236	5	NULL	NULL	0	NULL	reference model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In each of these four models , only one input variable ( concentration or bioavailability ) was changed compared with a reference model .
	manualset3
98827	1	400237	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In each treatment 20-kg portions of slurry ( n = 4 ) were stored for 95 d. All samples were subsampled nine to 10 times for determination of NH ( 3 ) and CH ( 4 ) evolution rates using a 2-L flow-through system .
	manualset3
98828	2	400237	5	NULL	NULL	0	NULL	20-kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In each treatment 20-kg portions of slurry ( n = 4 ) were stored for 95 d. All samples were subsampled nine to 10 times for determination of NH ( 3 ) and CH ( 4 ) evolution rates using a 2-L flow-through system .
	manualset3
98829	3	400237	5	NULL	NULL	0	NULL	portions 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In each treatment 20-kg portions of slurry ( n = 4 ) were stored for 95 d. All samples were subsampled nine to 10 times for determination of NH ( 3 ) and CH ( 4 ) evolution rates using a 2-L flow-through system .
	manualset3
98830	4	400237	5	NULL	NULL	0	NULL	slurry 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In each treatment 20-kg portions of slurry ( n = 4 ) were stored for 95 d. All samples were subsampled nine to 10 times for determination of NH ( 3 ) and CH ( 4 ) evolution rates using a 2-L flow-through system .
	manualset3
98831	5	400237	5	NULL	NULL	0	NULL	n = 4	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In each treatment 20-kg portions of slurry ( n = 4 ) were stored for 95 d. All samples were subsampled nine to 10 times for determination of NH ( 3 ) and CH ( 4 ) evolution rates using a 2-L flow-through system .
	manualset3
98832	6	400237	5	NULL	NULL	0	NULL	95 d	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In each treatment 20-kg portions of slurry ( n = 4 ) were stored for 95 d. All samples were subsampled nine to 10 times for determination of NH ( 3 ) and CH ( 4 ) evolution rates using a 2-L flow-through system .
	manualset3
98833	7	400237	5	NULL	NULL	0	NULL	samples	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In each treatment 20-kg portions of slurry ( n = 4 ) were stored for 95 d. All samples were subsampled nine to 10 times for determination of NH ( 3 ) and CH ( 4 ) evolution rates using a 2-L flow-through system .
	manualset3
98834	8	400237	5	NULL	NULL	0	NULL	nine to 10 times	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In each treatment 20-kg portions of slurry ( n = 4 ) were stored for 95 d. All samples were subsampled nine to 10 times for determination of NH ( 3 ) and CH ( 4 ) evolution rates using a 2-L flow-through system .
	manualset3
98835	9	400237	5	NULL	NULL	0	NULL	determination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In each treatment 20-kg portions of slurry ( n = 4 ) were stored for 95 d. All samples were subsampled nine to 10 times for determination of NH ( 3 ) and CH ( 4 ) evolution rates using a 2-L flow-through system .
	manualset3
98836	10	400237	5	NULL	NULL	0	NULL	NH ( 3 ) evolution rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In each treatment 20-kg portions of slurry ( n = 4 ) were stored for 95 d. All samples were subsampled nine to 10 times for determination of NH ( 3 ) and CH ( 4 ) evolution rates using a 2-L flow-through system .
	manualset3
98837	11	400237	5	NULL	NULL	0	NULL	CH ( 4 ) evolution rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In each treatment 20-kg portions of slurry ( n = 4 ) were stored for 95 d. All samples were subsampled nine to 10 times for determination of NH ( 3 ) and CH ( 4 ) evolution rates using a 2-L flow-through system .
	manualset3
98838	12	400237	5	NULL	NULL	0	NULL	2-L flow-through system	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In each treatment 20-kg portions of slurry ( n = 4 ) were stored for 95 d. All samples were subsampled nine to 10 times for determination of NH ( 3 ) and CH ( 4 ) evolution rates using a 2-L flow-through system .
	manualset3
98839	1	400238	5	NULL	NULL	NULL	NULL	early gestation ( G7 )	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In early gestation ( G7 ) , no change in hypothalamic neuropeptide Y ( NPY ) , agouti-related peptide ( AgRP ) , or proopiomelanocortin ( POMC ) expression was shown .
	manualset3
98840	2	400238	5	NULL	NULL	NULL	NULL	hypothalamic neuropeptide Y ( NPY )  expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In early gestation ( G7 ) , no change in hypothalamic neuropeptide Y ( NPY ) , agouti-related peptide ( AgRP ) , or proopiomelanocortin ( POMC ) expression was shown .
	manualset3
98841	3	400238	5	NULL	NULL	0	NULL	agouti-related peptide ( AgRP ) expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In early gestation ( G7 ) , no change in hypothalamic neuropeptide Y ( NPY ) , agouti-related peptide ( AgRP ) , or proopiomelanocortin ( POMC ) expression was shown .
	manualset3
98842	4	400238	5	NULL	NULL	0	NULL	proopiomelanocortin ( POMC ) expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In early gestation ( G7 ) , no change in hypothalamic neuropeptide Y ( NPY ) , agouti-related peptide ( AgRP ) , or proopiomelanocortin ( POMC ) expression was shown .
	manualset3
98843	1	400239	5	NULL	NULL	0	NULL	case	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In either case , greatest pain provocation will be associated with movements and functions in the sagittal plane .
	manualset3
98844	2	400239	5	NULL	NULL	0	NULL	greatest pain provocation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In either case , greatest pain provocation will be associated with movements and functions in the sagittal plane .
	manualset3
98845	3	400239	5	NULL	NULL	0	NULL	movements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In either case , greatest pain provocation will be associated with movements and functions in the sagittal plane .
	manualset3
98846	4	400239	5	NULL	NULL	0	NULL	functions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In either case , greatest pain provocation will be associated with movements and functions in the sagittal plane .
	manualset3
98847	5	400239	5	NULL	NULL	0	NULL	sagittal plane	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In either case , greatest pain provocation will be associated with movements and functions in the sagittal plane .
	manualset3
98848	1	400240	5	NULL	NULL	0	NULL	elderly hypertensives	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In elderly hypertensives with elevated serum cholesterol , differing risks have been reported .
	manualset3
98849	2	400240	5	NULL	NULL	NULL	NULL	elevated serum cholesterol	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In elderly hypertensives with elevated serum cholesterol , differing risks have been reported .
	manualset3
98850	3	400240	5	NULL	NULL	0	NULL	risks	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In elderly hypertensives with elevated serum cholesterol , differing risks have been reported .
	manualset3
98851	1	400241	5	NULL	NULL	0	NULL	electrophysiological experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In electrophysiological experiments in the same rats , thoracic spinal cord neurons responded dose-dependently to the mixture and , except for one neuron , responded also to BK in a dose-dependent manner .
	manualset3
98852	2	400241	5	NULL	NULL	0	NULL	rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In electrophysiological experiments in the same rats , thoracic spinal cord neurons responded dose-dependently to the mixture and , except for one neuron , responded also to BK in a dose-dependent manner .
	manualset3
98853	3	400241	5	NULL	NULL	0	NULL	thoracic spinal cord neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In electrophysiological experiments in the same rats , thoracic spinal cord neurons responded dose-dependently to the mixture and , except for one neuron , responded also to BK in a dose-dependent manner .
	manualset3
98854	4	400241	5	NULL	NULL	0	NULL	mixture	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In electrophysiological experiments in the same rats , thoracic spinal cord neurons responded dose-dependently to the mixture and , except for one neuron , responded also to BK in a dose-dependent manner .
	manualset3
98855	5	400241	5	NULL	NULL	0	NULL	neuron	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In electrophysiological experiments in the same rats , thoracic spinal cord neurons responded dose-dependently to the mixture and , except for one neuron , responded also to BK in a dose-dependent manner .
	manualset3
98856	6	400241	5	NULL	NULL	NULL	NULL	BK	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In electrophysiological experiments in the same rats , thoracic spinal cord neurons responded dose-dependently to the mixture and , except for one neuron , responded also to BK in a dose-dependent manner .
	manualset3
98857	1	400242	5	NULL	NULL	0	NULL	ethanol-treated rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In ethanol-treated rats , TRI exposure increased both the in vitro metabolism of TRI and the low-Km BAH activity but did not cause an apparent decrease in cytochrome P450 content even in animals with severe hepatic damage .
	manualset3
98858	2	400242	5	NULL	NULL	0	NULL	TRI exposure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In ethanol-treated rats , TRI exposure increased both the in vitro metabolism of TRI and the low-Km BAH activity but did not cause an apparent decrease in cytochrome P450 content even in animals with severe hepatic damage .
	manualset3
98859	3	400242	5	NULL	NULL	0	NULL	in vitro metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In ethanol-treated rats , TRI exposure increased both the in vitro metabolism of TRI and the low-Km BAH activity but did not cause an apparent decrease in cytochrome P450 content even in animals with severe hepatic damage .
	manualset3
98860	4	400242	5	NULL	NULL	0	NULL	TRI	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In ethanol-treated rats , TRI exposure increased both the in vitro metabolism of TRI and the low-Km BAH activity but did not cause an apparent decrease in cytochrome P450 content even in animals with severe hepatic damage .
	manualset3
98861	5	400242	5	NULL	NULL	0	NULL	low-Km BAH activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In ethanol-treated rats , TRI exposure increased both the in vitro metabolism of TRI and the low-Km BAH activity but did not cause an apparent decrease in cytochrome P450 content even in animals with severe hepatic damage .
	manualset3
98862	6	400242	5	NULL	NULL	0	NULL	cytochrome P450 content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In ethanol-treated rats , TRI exposure increased both the in vitro metabolism of TRI and the low-Km BAH activity but did not cause an apparent decrease in cytochrome P450 content even in animals with severe hepatic damage .
	manualset3
98863	7	400242	5	NULL	NULL	0	NULL	animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In ethanol-treated rats , TRI exposure increased both the in vitro metabolism of TRI and the low-Km BAH activity but did not cause an apparent decrease in cytochrome P450 content even in animals with severe hepatic damage .
	manualset3
98864	8	400242	5	NULL	NULL	0	NULL	severe hepatic damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In ethanol-treated rats , TRI exposure increased both the in vitro metabolism of TRI and the low-Km BAH activity but did not cause an apparent decrease in cytochrome P450 content even in animals with severe hepatic damage .
	manualset3
98865	1	400243	5	NULL	NULL	NULL	NULL	euthyroidism	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In euthyroidism triamcinolone exerts the opposite effect on the behavior of FFA ( decline was smaller and shorter ) and phosphatemia ( decline was pronounced and persists for longer period ) .
	manualset3
98866	2	400243	5	NULL	NULL	0	NULL	triamcinolone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In euthyroidism triamcinolone exerts the opposite effect on the behavior of FFA ( decline was smaller and shorter ) and phosphatemia ( decline was pronounced and persists for longer period ) .
	manualset3
98867	3	400243	5	NULL	NULL	0	NULL	opposite effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In euthyroidism triamcinolone exerts the opposite effect on the behavior of FFA ( decline was smaller and shorter ) and phosphatemia ( decline was pronounced and persists for longer period ) .
	manualset3
98868	4	400243	5	NULL	NULL	0	NULL	behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In euthyroidism triamcinolone exerts the opposite effect on the behavior of FFA ( decline was smaller and shorter ) and phosphatemia ( decline was pronounced and persists for longer period ) .
	manualset3
98869	5	400243	5	NULL	NULL	0	NULL	FFA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In euthyroidism triamcinolone exerts the opposite effect on the behavior of FFA ( decline was smaller and shorter ) and phosphatemia ( decline was pronounced and persists for longer period ) .
	manualset3
98870	6	400243	5	NULL	NULL	0	NULL	phosphatemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In euthyroidism triamcinolone exerts the opposite effect on the behavior of FFA ( decline was smaller and shorter ) and phosphatemia ( decline was pronounced and persists for longer period ) .
	manualset3
98871	7	400243	5	NULL	NULL	0	NULL	longer period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In euthyroidism triamcinolone exerts the opposite effect on the behavior of FFA ( decline was smaller and shorter ) and phosphatemia ( decline was pronounced and persists for longer period ) .
	manualset3
98872	1	400244	5	NULL	NULL	0	NULL	child 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In evaluating a child with a suspected cervical spine injury , radiography may be supplemented with CT or MRI .
	manualset3
98873	2	400244	5	NULL	NULL	0	NULL	cervical spine injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In evaluating a child with a suspected cervical spine injury , radiography may be supplemented with CT or MRI .
	manualset3
98874	3	400244	5	NULL	NULL	0	NULL	radiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In evaluating a child with a suspected cervical spine injury , radiography may be supplemented with CT or MRI .
	manualset3
98875	4	400244	5	NULL	NULL	0	NULL	CT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In evaluating a child with a suspected cervical spine injury , radiography may be supplemented with CT or MRI .
	manualset3
98876	5	400244	5	NULL	NULL	0	NULL	MRI	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In evaluating a child with a suspected cervical spine injury , radiography may be supplemented with CT or MRI .
	manualset3
98877	1	400245	5	NULL	NULL	0	NULL	experiment 5	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In experiment 5 , the effect of POEC was studied by co-culturing them with oocytes before IVF to determine if monospermy was improved .
	manualset3
98878	2	400245	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In experiment 5 , the effect of POEC was studied by co-culturing them with oocytes before IVF to determine if monospermy was improved .
	manualset3
98879	3	400245	5	NULL	NULL	0	NULL	POEC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In experiment 5 , the effect of POEC was studied by co-culturing them with oocytes before IVF to determine if monospermy was improved .
	manualset3
98880	4	400245	5	NULL	NULL	0	NULL	oocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In experiment 5 , the effect of POEC was studied by co-culturing them with oocytes before IVF to determine if monospermy was improved .
	manualset3
98881	5	400245	5	NULL	NULL	NULL	NULL	IVF 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In experiment 5 , the effect of POEC was studied by co-culturing them with oocytes before IVF to determine if monospermy was improved .
	manualset3
98882	6	400245	5	NULL	NULL	0	NULL	monospermy 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In experiment 5 , the effect of POEC was studied by co-culturing them with oocytes before IVF to determine if monospermy was improved .
	manualset3
98883	1	400246	5	NULL	NULL	0	NULL	highly selected panel	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( a ) A highly selected panel of antigens can be routinely used .
	manualset3
98884	2	400246	5	NULL	NULL	0	NULL	antigens	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	( a ) A highly selected panel of antigens can be routinely used .
	manualset3
98885	1	400247	5	NULL	NULL	0	NULL	experimental small bowel obstruction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In experimental small bowel obstruction an increased proportion of smooth endoplasmic reticulum and an increased number of lysosomes were seen in many liver cells .
	manualset3
98886	2	400247	5	NULL	NULL	0	NULL	increased proportion	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In experimental small bowel obstruction an increased proportion of smooth endoplasmic reticulum and an increased number of lysosomes were seen in many liver cells .
	manualset3
98887	3	400247	5	NULL	NULL	0	NULL	smooth endoplasmic reticulum	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In experimental small bowel obstruction an increased proportion of smooth endoplasmic reticulum and an increased number of lysosomes were seen in many liver cells .
	manualset3
98888	4	400247	5	NULL	NULL	0	NULL	increased number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In experimental small bowel obstruction an increased proportion of smooth endoplasmic reticulum and an increased number of lysosomes were seen in many liver cells .
	manualset3
98889	5	400247	5	NULL	NULL	0	NULL	lysosomes 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In experimental small bowel obstruction an increased proportion of smooth endoplasmic reticulum and an increased number of lysosomes were seen in many liver cells .
	manualset3
98890	6	400247	5	NULL	NULL	0	NULL	liver cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In experimental small bowel obstruction an increased proportion of smooth endoplasmic reticulum and an increased number of lysosomes were seen in many liver cells .
	manualset3
98891	1	400248	5	NULL	NULL	0	NULL	experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In experiments on a stirred tank reactor and a continuous scrubbing column in laboratory-scale , H ( 2 ) S was absorbed from a gas stream containing large amounts of carbon dioxide ( CO ( 2 ) ) into an aqueous solution prepared from sodium hydroxide ( NaOH ) , sodium bicarbonate ( NaHCO ( 3 ) ) and hydrogen peroxide ( H ( 2 ) O ( 2 ) ) .
	manualset3
98892	2	400248	5	NULL	NULL	0	NULL	stirred tank reactor	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In experiments on a stirred tank reactor and a continuous scrubbing column in laboratory-scale , H ( 2 ) S was absorbed from a gas stream containing large amounts of carbon dioxide ( CO ( 2 ) ) into an aqueous solution prepared from sodium hydroxide ( NaOH ) , sodium bicarbonate ( NaHCO ( 3 ) ) and hydrogen peroxide ( H ( 2 ) O ( 2 ) ) .
	manualset3
98893	3	400248	5	NULL	NULL	0	NULL	continuous scrubbing column	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In experiments on a stirred tank reactor and a continuous scrubbing column in laboratory-scale , H ( 2 ) S was absorbed from a gas stream containing large amounts of carbon dioxide ( CO ( 2 ) ) into an aqueous solution prepared from sodium hydroxide ( NaOH ) , sodium bicarbonate ( NaHCO ( 3 ) ) and hydrogen peroxide ( H ( 2 ) O ( 2 ) ) .
	manualset3
98894	4	400248	5	NULL	NULL	0	NULL	laboratory-scale	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In experiments on a stirred tank reactor and a continuous scrubbing column in laboratory-scale , H ( 2 ) S was absorbed from a gas stream containing large amounts of carbon dioxide ( CO ( 2 ) ) into an aqueous solution prepared from sodium hydroxide ( NaOH ) , sodium bicarbonate ( NaHCO ( 3 ) ) and hydrogen peroxide ( H ( 2 ) O ( 2 ) ) .
	manualset3
98895	5	400248	5	NULL	NULL	NULL	NULL	H ( 2 ) S	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In experiments on a stirred tank reactor and a continuous scrubbing column in laboratory-scale , H ( 2 ) S was absorbed from a gas stream containing large amounts of carbon dioxide ( CO ( 2 ) ) into an aqueous solution prepared from sodium hydroxide ( NaOH ) , sodium bicarbonate ( NaHCO ( 3 ) ) and hydrogen peroxide ( H ( 2 ) O ( 2 ) ) .
	manualset3
98896	6	400248	5	NULL	NULL	NULL	NULL	gas stream	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In experiments on a stirred tank reactor and a continuous scrubbing column in laboratory-scale , H ( 2 ) S was absorbed from a gas stream containing large amounts of carbon dioxide ( CO ( 2 ) ) into an aqueous solution prepared from sodium hydroxide ( NaOH ) , sodium bicarbonate ( NaHCO ( 3 ) ) and hydrogen peroxide ( H ( 2 ) O ( 2 ) ) .
	manualset3
98897	7	400248	5	NULL	NULL	0	NULL	large amounts 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In experiments on a stirred tank reactor and a continuous scrubbing column in laboratory-scale , H ( 2 ) S was absorbed from a gas stream containing large amounts of carbon dioxide ( CO ( 2 ) ) into an aqueous solution prepared from sodium hydroxide ( NaOH ) , sodium bicarbonate ( NaHCO ( 3 ) ) and hydrogen peroxide ( H ( 2 ) O ( 2 ) ) .
	manualset3
98898	8	400248	5	NULL	NULL	NULL	NULL	( CO ( 2 ) )	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In experiments on a stirred tank reactor and a continuous scrubbing column in laboratory-scale , H ( 2 ) S was absorbed from a gas stream containing large amounts of carbon dioxide ( CO ( 2 ) ) into an aqueous solution prepared from sodium hydroxide ( NaOH ) , sodium bicarbonate ( NaHCO ( 3 ) ) and hydrogen peroxide ( H ( 2 ) O ( 2 ) ) .
	manualset3
98900	9	400248	5	NULL	NULL	0	NULL	aqueous solution	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In experiments on a stirred tank reactor and a continuous scrubbing column in laboratory-scale , H ( 2 ) S was absorbed from a gas stream containing large amounts of carbon dioxide ( CO ( 2 ) ) into an aqueous solution prepared from sodium hydroxide ( NaOH ) , sodium bicarbonate ( NaHCO ( 3 ) ) and hydrogen peroxide ( H ( 2 ) O ( 2 ) ) .
	manualset3
98901	10	400248	5	NULL	NULL	0	NULL	sodium hydroxide ( NaOH )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In experiments on a stirred tank reactor and a continuous scrubbing column in laboratory-scale , H ( 2 ) S was absorbed from a gas stream containing large amounts of carbon dioxide ( CO ( 2 ) ) into an aqueous solution prepared from sodium hydroxide ( NaOH ) , sodium bicarbonate ( NaHCO ( 3 ) ) and hydrogen peroxide ( H ( 2 ) O ( 2 ) ) .
	manualset3
98902	11	400248	5	NULL	NULL	0	NULL	sodium bicarbonate ( NaHCO ( 3 ) )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In experiments on a stirred tank reactor and a continuous scrubbing column in laboratory-scale , H ( 2 ) S was absorbed from a gas stream containing large amounts of carbon dioxide ( CO ( 2 ) ) into an aqueous solution prepared from sodium hydroxide ( NaOH ) , sodium bicarbonate ( NaHCO ( 3 ) ) and hydrogen peroxide ( H ( 2 ) O ( 2 ) ) .
	manualset3
98903	12	400248	5	NULL	NULL	0	NULL	hydrogen peroxide ( H ( 2 ) O ( 2 ) )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In experiments on a stirred tank reactor and a continuous scrubbing column in laboratory-scale , H ( 2 ) S was absorbed from a gas stream containing large amounts of carbon dioxide ( CO ( 2 ) ) into an aqueous solution prepared from sodium hydroxide ( NaOH ) , sodium bicarbonate ( NaHCO ( 3 ) ) and hydrogen peroxide ( H ( 2 ) O ( 2 ) ) .
	manualset3
98904	1	400249	5	NULL	NULL	0	NULL	extracts	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In extracts of both lungs and atria , high-performance liquid chromatography revealed two forms of the peptide ; prohormone and a carboxy-terminal peptide of low molecular mass , which is the biologically active form of peptide .
	manualset3
99069	2	400249	5	NULL	NULL	0	NULL	lungs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In extracts of both lungs and atria , high-performance liquid chromatography revealed two forms of the peptide ; prohormone and a carboxy-terminal peptide of low molecular mass , which is the biologically active form of peptide .
	manualset3
99070	3	400249	5	NULL	NULL	0	NULL	atria	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In extracts of both lungs and atria , high-performance liquid chromatography revealed two forms of the peptide ; prohormone and a carboxy-terminal peptide of low molecular mass , which is the biologically active form of peptide .
	manualset3
99071	4	400249	5	NULL	NULL	0	NULL	high-performance liquid chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In extracts of both lungs and atria , high-performance liquid chromatography revealed two forms of the peptide ; prohormone and a carboxy-terminal peptide of low molecular mass , which is the biologically active form of peptide .
	manualset3
99072	5	400249	5	NULL	NULL	0	NULL	two forms of the peptide	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In extracts of both lungs and atria , high-performance liquid chromatography revealed two forms of the peptide ; prohormone and a carboxy-terminal peptide of low molecular mass , which is the biologically active form of peptide .
	manualset3
99073	6	400249	5	NULL	NULL	0	NULL	prohormone	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In extracts of both lungs and atria , high-performance liquid chromatography revealed two forms of the peptide ; prohormone and a carboxy-terminal peptide of low molecular mass , which is the biologically active form of peptide .
	manualset3
99074	7	400249	5	NULL	NULL	NULL	NULL	carboxy-terminal peptide	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In extracts of both lungs and atria , high-performance liquid chromatography revealed two forms of the peptide ; prohormone and a carboxy-terminal peptide of low molecular mass , which is the biologically active form of peptide .
	manualset3
99075	8	400249	5	NULL	NULL	0	NULL	low molecular mass	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In extracts of both lungs and atria , high-performance liquid chromatography revealed two forms of the peptide ; prohormone and a carboxy-terminal peptide of low molecular mass , which is the biologically active form of peptide .
	manualset3
99076	9	400249	5	NULL	NULL	0	NULL	biologically active form of peptide	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In extracts of both lungs and atria , high-performance liquid chromatography revealed two forms of the peptide ; prohormone and a carboxy-terminal peptide of low molecular mass , which is the biologically active form of peptide .
	manualset3
99077	1	400250	5	NULL	NULL	0	NULL	eyes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In eyes with increased intraocular pressure , these values were 12.2 + / - 1.2 C.U. Moreover , the amount of norepinephrine in tissue homogenates of the same eyes was evaluated and found to be 21.7 + / - 1.3 microg/gr tissue fresh weight of the human uveoscleral tissue in eyes with normal intraocular pressure .
	manualset3
99078	2	400250	5	NULL	NULL	0	NULL	increased intraocular pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In eyes with increased intraocular pressure , these values were 12.2 + / - 1.2 C.U. Moreover , the amount of norepinephrine in tissue homogenates of the same eyes was evaluated and found to be 21.7 + / - 1.3 microg/gr tissue fresh weight of the human uveoscleral tissue in eyes with normal intraocular pressure .
	manualset3
99079	3	400250	5	NULL	NULL	0	NULL	values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In eyes with increased intraocular pressure , these values were 12.2 + / - 1.2 C.U. Moreover , the amount of norepinephrine in tissue homogenates of the same eyes was evaluated and found to be 21.7 + / - 1.3 microg/gr tissue fresh weight of the human uveoscleral tissue in eyes with normal intraocular pressure .
	manualset3
99080	4	400250	5	NULL	NULL	0	NULL	12.2 + / - 1.2 C.U	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In eyes with increased intraocular pressure , these values were 12.2 + / - 1.2 C.U. Moreover , the amount of norepinephrine in tissue homogenates of the same eyes was evaluated and found to be 21.7 + / - 1.3 microg/gr tissue fresh weight of the human uveoscleral tissue in eyes with normal intraocular pressure .
	manualset3
99081	5	400250	5	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In eyes with increased intraocular pressure , these values were 12.2 + / - 1.2 C.U. Moreover , the amount of norepinephrine in tissue homogenates of the same eyes was evaluated and found to be 21.7 + / - 1.3 microg/gr tissue fresh weight of the human uveoscleral tissue in eyes with normal intraocular pressure .
	manualset3
99082	6	400250	5	NULL	NULL	NULL	NULL	norepinephrine	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In eyes with increased intraocular pressure , these values were 12.2 + / - 1.2 C.U. Moreover , the amount of norepinephrine in tissue homogenates of the same eyes was evaluated and found to be 21.7 + / - 1.3 microg/gr tissue fresh weight of the human uveoscleral tissue in eyes with normal intraocular pressure .
	manualset3
99083	7	400250	5	NULL	NULL	0	NULL	tissue homogenates	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In eyes with increased intraocular pressure , these values were 12.2 + / - 1.2 C.U. Moreover , the amount of norepinephrine in tissue homogenates of the same eyes was evaluated and found to be 21.7 + / - 1.3 microg/gr tissue fresh weight of the human uveoscleral tissue in eyes with normal intraocular pressure .
	manualset3
99084	8	400250	5	NULL	NULL	0	NULL	same eyes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In eyes with increased intraocular pressure , these values were 12.2 + / - 1.2 C.U. Moreover , the amount of norepinephrine in tissue homogenates of the same eyes was evaluated and found to be 21.7 + / - 1.3 microg/gr tissue fresh weight of the human uveoscleral tissue in eyes with normal intraocular pressure .
	manualset3
99085	9	400250	5	NULL	NULL	0	NULL	21.7 + / - 1.3 microg/gr	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In eyes with increased intraocular pressure , these values were 12.2 + / - 1.2 C.U. Moreover , the amount of norepinephrine in tissue homogenates of the same eyes was evaluated and found to be 21.7 + / - 1.3 microg/gr tissue fresh weight of the human uveoscleral tissue in eyes with normal intraocular pressure .
	manualset3
99086	10	400250	5	NULL	NULL	0	NULL	tissue fresh weight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In eyes with increased intraocular pressure , these values were 12.2 + / - 1.2 C.U. Moreover , the amount of norepinephrine in tissue homogenates of the same eyes was evaluated and found to be 21.7 + / - 1.3 microg/gr tissue fresh weight of the human uveoscleral tissue in eyes with normal intraocular pressure .
	manualset3
99087	11	400250	5	NULL	NULL	0	NULL	human uveoscleral tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In eyes with increased intraocular pressure , these values were 12.2 + / - 1.2 C.U. Moreover , the amount of norepinephrine in tissue homogenates of the same eyes was evaluated and found to be 21.7 + / - 1.3 microg/gr tissue fresh weight of the human uveoscleral tissue in eyes with normal intraocular pressure .
	manualset3
99088	12	400250	5	NULL	NULL	0	NULL	eyes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In eyes with increased intraocular pressure , these values were 12.2 + / - 1.2 C.U. Moreover , the amount of norepinephrine in tissue homogenates of the same eyes was evaluated and found to be 21.7 + / - 1.3 microg/gr tissue fresh weight of the human uveoscleral tissue in eyes with normal intraocular pressure .
	manualset3
99089	13	400250	5	NULL	NULL	0	NULL	normal intraocular pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In eyes with increased intraocular pressure , these values were 12.2 + / - 1.2 C.U. Moreover , the amount of norepinephrine in tissue homogenates of the same eyes was evaluated and found to be 21.7 + / - 1.3 microg/gr tissue fresh weight of the human uveoscleral tissue in eyes with normal intraocular pressure .
	manualset3
99090	1	400251	5	NULL	NULL	0	NULL	families	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In families which had a history of unemployment or unskilled occupations , adults and informal carers were most likely to treat certain hazards as risks to be taken .
	manualset3
99091	2	400251	5	NULL	NULL	0	NULL	history	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In families which had a history of unemployment or unskilled occupations , adults and informal carers were most likely to treat certain hazards as risks to be taken .
	manualset3
99092	3	400251	5	NULL	NULL	0	NULL	unemployment	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In families which had a history of unemployment or unskilled occupations , adults and informal carers were most likely to treat certain hazards as risks to be taken .
	manualset3
99093	4	400251	5	NULL	NULL	0	NULL	unskilled occupations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In families which had a history of unemployment or unskilled occupations , adults and informal carers were most likely to treat certain hazards as risks to be taken .
	manualset3
99094	5	400251	5	NULL	NULL	0	NULL	adults 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In families which had a history of unemployment or unskilled occupations , adults and informal carers were most likely to treat certain hazards as risks to be taken .
	manualset3
99095	6	400251	5	NULL	NULL	0	NULL	informal carers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In families which had a history of unemployment or unskilled occupations , adults and informal carers were most likely to treat certain hazards as risks to be taken .
	manualset3
99096	7	400251	5	NULL	NULL	0	NULL	treat	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In families which had a history of unemployment or unskilled occupations , adults and informal carers were most likely to treat certain hazards as risks to be taken .
	manualset3
99097	8	400251	5	NULL	NULL	NULL	NULL	hazards	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In families which had a history of unemployment or unskilled occupations , adults and informal carers were most likely to treat certain hazards as risks to be taken .
	manualset3
99098	9	400251	5	NULL	NULL	0	NULL	risks	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In families which had a history of unemployment or unskilled occupations , adults and informal carers were most likely to treat certain hazards as risks to be taken .
	manualset3
99099	1	400252	5	NULL	NULL	0	NULL	filamentous fungi	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In filamentous fungi , a cell death reaction known as an incompatibility reaction occurs when cells of unlike genotype fuse .
	manualset3
99100	2	400252	5	NULL	NULL	0	NULL	cell death reaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In filamentous fungi , a cell death reaction known as an incompatibility reaction occurs when cells of unlike genotype fuse .
	manualset3
99101	3	400252	5	NULL	NULL	0	NULL	incompatibility reaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In filamentous fungi , a cell death reaction known as an incompatibility reaction occurs when cells of unlike genotype fuse .
	manualset3
99102	4	400252	5	NULL	NULL	0	NULL	cells of unlike genotype 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In filamentous fungi , a cell death reaction known as an incompatibility reaction occurs when cells of unlike genotype fuse .
	manualset3
99103	1	400253	5	NULL	NULL	0	NULL	fit candidates	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In fit candidates with potentially resectable lesions , the authors eschew pre - or intraoperative biopsy , angiography , or endoscopic stenting and use preliminary limited staging laparoscopy selectively .
	manualset3
99104	2	400253	5	NULL	NULL	0	NULL	potentially resectable lesions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In fit candidates with potentially resectable lesions , the authors eschew pre - or intraoperative biopsy , angiography , or endoscopic stenting and use preliminary limited staging laparoscopy selectively .
	manualset3
99105	3	400253	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In fit candidates with potentially resectable lesions , the authors eschew pre - or intraoperative biopsy , angiography , or endoscopic stenting and use preliminary limited staging laparoscopy selectively .
	manualset3
99106	4	400253	5	NULL	NULL	0	NULL	pre - or intraoperative biopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In fit candidates with potentially resectable lesions , the authors eschew pre - or intraoperative biopsy , angiography , or endoscopic stenting and use preliminary limited staging laparoscopy selectively .
	manualset3
99107	5	400253	5	NULL	NULL	0	NULL	angiography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In fit candidates with potentially resectable lesions , the authors eschew pre - or intraoperative biopsy , angiography , or endoscopic stenting and use preliminary limited staging laparoscopy selectively .
	manualset3
99108	6	400253	5	NULL	NULL	0	NULL	endoscopic stenting	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In fit candidates with potentially resectable lesions , the authors eschew pre - or intraoperative biopsy , angiography , or endoscopic stenting and use preliminary limited staging laparoscopy selectively .
	manualset3
99109	7	400253	5	NULL	NULL	0	NULL	preliminary limited staging laparoscopy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In fit candidates with potentially resectable lesions , the authors eschew pre - or intraoperative biopsy , angiography , or endoscopic stenting and use preliminary limited staging laparoscopy selectively .
	manualset3
99110	1	400254	5	NULL	NULL	0	NULL	five cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In five cases additional clusters were also found by the detector .
	manualset3
99111	2	400254	5	NULL	NULL	0	NULL	additional clusters	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In five cases additional clusters were also found by the detector .
	manualset3
99112	3	400254	5	NULL	NULL	0	NULL	detector	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In five cases additional clusters were also found by the detector .
	manualset3
99113	1	400255	5	NULL	NULL	0	NULL	four cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In four cases the immunoglobulin heavy chain gene polymerase chain study revealed the same rearrangement pattern in both primary and secondary tumors , thereby confirming their identity and excluding the possibility of a second malignancy .
	manualset3
99114	2	400255	5	NULL	NULL	0	NULL	immunoglobulin heavy chain gene polymerase chain study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In four cases the immunoglobulin heavy chain gene polymerase chain study revealed the same rearrangement pattern in both primary and secondary tumors , thereby confirming their identity and excluding the possibility of a second malignancy .
	manualset3
99115	3	400255	5	NULL	NULL	0	NULL	same rearrangement pattern	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In four cases the immunoglobulin heavy chain gene polymerase chain study revealed the same rearrangement pattern in both primary and secondary tumors , thereby confirming their identity and excluding the possibility of a second malignancy .
	manualset3
99116	4	400255	5	NULL	NULL	0	NULL	primary and secondary tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In four cases the immunoglobulin heavy chain gene polymerase chain study revealed the same rearrangement pattern in both primary and secondary tumors , thereby confirming their identity and excluding the possibility of a second malignancy .
	manualset3
99117	5	400255	5	NULL	NULL	0	NULL	identity 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In four cases the immunoglobulin heavy chain gene polymerase chain study revealed the same rearrangement pattern in both primary and secondary tumors , thereby confirming their identity and excluding the possibility of a second malignancy .
	manualset3
99118	6	400255	5	NULL	NULL	0	NULL	second malignancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In four cases the immunoglobulin heavy chain gene polymerase chain study revealed the same rearrangement pattern in both primary and secondary tumors , thereby confirming their identity and excluding the possibility of a second malignancy .
	manualset3
99119	1	400256	5	NULL	NULL	0	NULL	 four experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In four experiments , listeners ' response times to detect vowel targets in spoken input were measured .
	manualset3
99120	2	400256	5	NULL	NULL	0	NULL	listeners ' response times	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In four experiments , listeners ' response times to detect vowel targets in spoken input were measured .
	manualset3
99121	3	400256	5	NULL	NULL	NULL	NULL	vowel targets in spoken input	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In four experiments , listeners ' response times to detect vowel targets in spoken input were measured .
	manualset3
99122	1	400257	5	NULL	NULL	0	NULL	four well designed , phase II or III trials ( RESOLVE , RESTORE , RIDE and RISE ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In four well designed , phase II or III trials ( RESOLVE , RESTORE , RIDE and RISE ) , 1-2 years ' treatment with ranibizumab was more effective than sham or focal/grid laser therapy in improving best corrected visual acuity ( BCVA ) and reducing central retinal thickness ( CRT ) in patients with visual impairment associated with DME .
	manualset3
99123	2	400257	5	NULL	NULL	0	NULL	1-2 years	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In four well designed , phase II or III trials ( RESOLVE , RESTORE , RIDE and RISE ) , 1-2 years ' treatment with ranibizumab was more effective than sham or focal/grid laser therapy in improving best corrected visual acuity ( BCVA ) and reducing central retinal thickness ( CRT ) in patients with visual impairment associated with DME .
	manualset3
99124	3	400257	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In four well designed , phase II or III trials ( RESOLVE , RESTORE , RIDE and RISE ) , 1-2 years ' treatment with ranibizumab was more effective than sham or focal/grid laser therapy in improving best corrected visual acuity ( BCVA ) and reducing central retinal thickness ( CRT ) in patients with visual impairment associated with DME .
	manualset3
99125	4	400257	5	NULL	NULL	0	NULL	ranibizumab 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In four well designed , phase II or III trials ( RESOLVE , RESTORE , RIDE and RISE ) , 1-2 years ' treatment with ranibizumab was more effective than sham or focal/grid laser therapy in improving best corrected visual acuity ( BCVA ) and reducing central retinal thickness ( CRT ) in patients with visual impairment associated with DME .
	manualset3
99126	5	400257	5	NULL	NULL	0	NULL	sham or focal/grid laser therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In four well designed , phase II or III trials ( RESOLVE , RESTORE , RIDE and RISE ) , 1-2 years ' treatment with ranibizumab was more effective than sham or focal/grid laser therapy in improving best corrected visual acuity ( BCVA ) and reducing central retinal thickness ( CRT ) in patients with visual impairment associated with DME .
	manualset3
99127	6	400257	5	NULL	NULL	NULL	NULL	best corrected visual acuity ( BCVA )	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In four well designed , phase II or III trials ( RESOLVE , RESTORE , RIDE and RISE ) , 1-2 years ' treatment with ranibizumab was more effective than sham or focal/grid laser therapy in improving best corrected visual acuity ( BCVA ) and reducing central retinal thickness ( CRT ) in patients with visual impairment associated with DME .
	manualset3
99128	7	400257	5	NULL	NULL	0	NULL	central retinal thickness ( CRT )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In four well designed , phase II or III trials ( RESOLVE , RESTORE , RIDE and RISE ) , 1-2 years ' treatment with ranibizumab was more effective than sham or focal/grid laser therapy in improving best corrected visual acuity ( BCVA ) and reducing central retinal thickness ( CRT ) in patients with visual impairment associated with DME .
	manualset3
99129	8	400257	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In four well designed , phase II or III trials ( RESOLVE , RESTORE , RIDE and RISE ) , 1-2 years ' treatment with ranibizumab was more effective than sham or focal/grid laser therapy in improving best corrected visual acuity ( BCVA ) and reducing central retinal thickness ( CRT ) in patients with visual impairment associated with DME .
	manualset3
99130	9	400257	5	NULL	NULL	0	NULL	visual impairment associated with DME	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In four well designed , phase II or III trials ( RESOLVE , RESTORE , RIDE and RISE ) , 1-2 years ' treatment with ranibizumab was more effective than sham or focal/grid laser therapy in improving best corrected visual acuity ( BCVA ) and reducing central retinal thickness ( CRT ) in patients with visual impairment associated with DME .
	manualset3
99131	1	400258	5	NULL	NULL	0	NULL	consequential injurious role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In further support of the consequential injurious role of oxidative stress , many of the adverse effects of high glucose on endothelial functions , such as reduced endothelial-dependent relaxation and delayed cell replication , are reversed by antioxidants .
	manualset3
99132	2	400258	5	NULL	NULL	0	NULL	oxidative stress	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In further support of the consequential injurious role of oxidative stress , many of the adverse effects of high glucose on endothelial functions , such as reduced endothelial-dependent relaxation and delayed cell replication , are reversed by antioxidants .
	manualset3
99133	3	400258	5	NULL	NULL	0	NULL	adverse effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In further support of the consequential injurious role of oxidative stress , many of the adverse effects of high glucose on endothelial functions , such as reduced endothelial-dependent relaxation and delayed cell replication , are reversed by antioxidants .
	manualset3
99134	4	400258	5	NULL	NULL	0	NULL	high glucose	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In further support of the consequential injurious role of oxidative stress , many of the adverse effects of high glucose on endothelial functions , such as reduced endothelial-dependent relaxation and delayed cell replication , are reversed by antioxidants .
	manualset3
99135	5	400258	5	NULL	NULL	0	NULL	endothelial functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In further support of the consequential injurious role of oxidative stress , many of the adverse effects of high glucose on endothelial functions , such as reduced endothelial-dependent relaxation and delayed cell replication , are reversed by antioxidants .
	manualset3
99136	6	400258	5	NULL	NULL	0	NULL	reduced endothelial-dependent relaxation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In further support of the consequential injurious role of oxidative stress , many of the adverse effects of high glucose on endothelial functions , such as reduced endothelial-dependent relaxation and delayed cell replication , are reversed by antioxidants .
	manualset3
99137	7	400258	5	NULL	NULL	0	NULL	delayed cell replication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In further support of the consequential injurious role of oxidative stress , many of the adverse effects of high glucose on endothelial functions , such as reduced endothelial-dependent relaxation and delayed cell replication , are reversed by antioxidants .
	manualset3
99138	8	400258	5	NULL	NULL	0	NULL	antioxidants 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In further support of the consequential injurious role of oxidative stress , many of the adverse effects of high glucose on endothelial functions , such as reduced endothelial-dependent relaxation and delayed cell replication , are reversed by antioxidants .
	manualset3
99139	1	400259	5	NULL	NULL	0	NULL	4-nitrophenol glucuronidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In general 4-nitrophenol glucuronidation was more effectively inhibited than that of 1-naphthol , bilirubin or testosterone .
	manualset3
99140	2	400259	5	NULL	NULL	0	NULL	1-naphthol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In general 4-nitrophenol glucuronidation was more effectively inhibited than that of 1-naphthol , bilirubin or testosterone .
	manualset3
99141	3	400259	5	NULL	NULL	0	NULL	bilirubin	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In general 4-nitrophenol glucuronidation was more effectively inhibited than that of 1-naphthol , bilirubin or testosterone .
	manualset3
99142	4	400259	5	NULL	NULL	0	NULL	testosterone 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In general 4-nitrophenol glucuronidation was more effectively inhibited than that of 1-naphthol , bilirubin or testosterone .
	manualset3
99389	1	400260	5	NULL	NULL	0	NULL	LA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In general we have found LA and COA as simple , rapid specific and sensitive tests and can be applied even in field situations and that LA can be used for antigen detection in urine and IEOP in serum .
	manualset3
99390	2	400260	5	NULL	NULL	0	NULL	COA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In general we have found LA and COA as simple , rapid specific and sensitive tests and can be applied even in field situations and that LA can be used for antigen detection in urine and IEOP in serum .
	manualset3
99394	3	400260	5	NULL	NULL	0	NULL	rapid specific and sensitive tests	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In general we have found LA and COA as simple , rapid specific and sensitive tests and can be applied even in field situations and that LA can be used for antigen detection in urine and IEOP in serum .
	manualset3
99396	4	400260	5	NULL	NULL	0	NULL	field situations	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In general we have found LA and COA as simple , rapid specific and sensitive tests and can be applied even in field situations and that LA can be used for antigen detection in urine and IEOP in serum .
	manualset3
99397	5	400260	5	NULL	NULL	0	NULL	LA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In general we have found LA and COA as simple , rapid specific and sensitive tests and can be applied even in field situations and that LA can be used for antigen detection in urine and IEOP in serum .
	manualset3
99398	6	400260	5	NULL	NULL	0	NULL	antigen detection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In general we have found LA and COA as simple , rapid specific and sensitive tests and can be applied even in field situations and that LA can be used for antigen detection in urine and IEOP in serum .
	manualset3
99400	7	400260	5	NULL	NULL	0	NULL	urine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In general we have found LA and COA as simple , rapid specific and sensitive tests and can be applied even in field situations and that LA can be used for antigen detection in urine and IEOP in serum .
	manualset3
99403	8	400260	5	NULL	NULL	0	NULL	IEOP	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In general we have found LA and COA as simple , rapid specific and sensitive tests and can be applied even in field situations and that LA can be used for antigen detection in urine and IEOP in serum .
	manualset3
99404	9	400260	5	NULL	NULL	0	NULL	serum	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In general we have found LA and COA as simple , rapid specific and sensitive tests and can be applied even in field situations and that LA can be used for antigen detection in urine and IEOP in serum .
	manualset3
99405	1	400261	5	NULL	NULL	0	NULL	gill tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In gill tissue of IPW-acclimated goldfish , transcript abundance of tight junction ( TJ ) proteins occludin , claudin-b , - d , - e , - h , -7 , and -8 d increased , whereas ZO-1 and claudin 12 mRNA decreased and claudin-c was unaltered .
	manualset3
99406	2	400261	5	NULL	NULL	0	NULL	IPW-acclimated goldfish	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In gill tissue of IPW-acclimated goldfish , transcript abundance of tight junction ( TJ ) proteins occludin , claudin-b , - d , - e , - h , -7 , and -8 d increased , whereas ZO-1 and claudin 12 mRNA decreased and claudin-c was unaltered .
	manualset3
99408	3	400261	5	NULL	NULL	0	NULL	transcript abundance	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In gill tissue of IPW-acclimated goldfish , transcript abundance of tight junction ( TJ ) proteins occludin , claudin-b , - d , - e , - h , -7 , and -8 d increased , whereas ZO-1 and claudin 12 mRNA decreased and claudin-c was unaltered .
	manualset3
99409	4	400261	5	NULL	NULL	0	NULL	tight junction ( TJ ) proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In gill tissue of IPW-acclimated goldfish , transcript abundance of tight junction ( TJ ) proteins occludin , claudin-b , - d , - e , - h , -7 , and -8 d increased , whereas ZO-1 and claudin 12 mRNA decreased and claudin-c was unaltered .
	manualset3
99410	5	400261	5	NULL	NULL	0	NULL	occludin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In gill tissue of IPW-acclimated goldfish , transcript abundance of tight junction ( TJ ) proteins occludin , claudin-b , - d , - e , - h , -7 , and -8 d increased , whereas ZO-1 and claudin 12 mRNA decreased and claudin-c was unaltered .
	manualset3
99411	6	400261	5	NULL	NULL	0	NULL	claudin-b	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In gill tissue of IPW-acclimated goldfish , transcript abundance of tight junction ( TJ ) proteins occludin , claudin-b , - d , - e , - h , -7 , and -8 d increased , whereas ZO-1 and claudin 12 mRNA decreased and claudin-c was unaltered .
	manualset3
99412	7	400261	5	NULL	NULL	0	NULL	claudin-d	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In gill tissue of IPW-acclimated goldfish , transcript abundance of tight junction ( TJ ) proteins occludin , claudin-b , - d , - e , - h , -7 , and -8 d increased , whereas ZO-1 and claudin 12 mRNA decreased and claudin-c was unaltered .
	manualset3
99413	8	400261	5	NULL	NULL	0	NULL	claudin-e	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In gill tissue of IPW-acclimated goldfish , transcript abundance of tight junction ( TJ ) proteins occludin , claudin-b , - d , - e , - h , -7 , and -8 d increased , whereas ZO-1 and claudin 12 mRNA decreased and claudin-c was unaltered .
	manualset3
99415	9	400261	5	NULL	NULL	0	NULL	claudin-h	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In gill tissue of IPW-acclimated goldfish , transcript abundance of tight junction ( TJ ) proteins occludin , claudin-b , - d , - e , - h , -7 , and -8 d increased , whereas ZO-1 and claudin 12 mRNA decreased and claudin-c was unaltered .
	manualset3
99417	10	400261	5	NULL	NULL	0	NULL	claudin-7	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In gill tissue of IPW-acclimated goldfish , transcript abundance of tight junction ( TJ ) proteins occludin , claudin-b , - d , - e , - h , -7 , and -8 d increased , whereas ZO-1 and claudin 12 mRNA decreased and claudin-c was unaltered .
	manualset3
99418	11	400261	5	NULL	NULL	0	NULL	claudin-8 d	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In gill tissue of IPW-acclimated goldfish , transcript abundance of tight junction ( TJ ) proteins occludin , claudin-b , - d , - e , - h , -7 , and -8 d increased , whereas ZO-1 and claudin 12 mRNA decreased and claudin-c was unaltered .
	manualset3
99421	12	400261	5	NULL	NULL	0	NULL	ZO-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In gill tissue of IPW-acclimated goldfish , transcript abundance of tight junction ( TJ ) proteins occludin , claudin-b , - d , - e , - h , -7 , and -8 d increased , whereas ZO-1 and claudin 12 mRNA decreased and claudin-c was unaltered .
	manualset3
99423	13	400261	5	NULL	NULL	0	NULL	claudin 12 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In gill tissue of IPW-acclimated goldfish , transcript abundance of tight junction ( TJ ) proteins occludin , claudin-b , - d , - e , - h , -7 , and -8 d increased , whereas ZO-1 and claudin 12 mRNA decreased and claudin-c was unaltered .
	manualset3
99424	14	400261	5	NULL	NULL	0	NULL	claudin-c	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In gill tissue of IPW-acclimated goldfish , transcript abundance of tight junction ( TJ ) proteins occludin , claudin-b , - d , - e , - h , -7 , and -8 d increased , whereas ZO-1 and claudin 12 mRNA decreased and claudin-c was unaltered .
	manualset3
99428	1	400262	5	NULL	NULL	0	NULL	gp130 ( Delta STAT/Delta STAT ) bone marrow-derived macrophages ( BMMs )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In gp130 ( Delta STAT/Delta STAT ) bone marrow-derived macrophages ( BMMs ) , both IL-6 - and M-CSF-induced ERK1/2 tyrosine phosphorylation was enhanced .
	manualset3
99429	2	400262	5	NULL	NULL	NULL	NULL	IL-6 -induced ERK1/2 tyrosine phosphorylation	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In gp130 ( Delta STAT/Delta STAT ) bone marrow-derived macrophages ( BMMs ) , both IL-6 - and M-CSF-induced ERK1/2 tyrosine phosphorylation was enhanced .
	manualset3
99430	3	400262	5	NULL	NULL	0	NULL	M-CSF-induced ERK1/2 tyrosine phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In gp130 ( Delta STAT/Delta STAT ) bone marrow-derived macrophages ( BMMs ) , both IL-6 - and M-CSF-induced ERK1/2 tyrosine phosphorylation was enhanced .
	manualset3
99431	1	400263	5	NULL	NULL	0	NULL	intimate relationship	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( d ) There is an intimate relationship between unexplained syncope and psychiatric illness , mandating a combined medical and psychiatric approach to such patients .
	manualset3
99432	2	400263	5	NULL	NULL	0	NULL	unexplained syncope	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( d ) There is an intimate relationship between unexplained syncope and psychiatric illness , mandating a combined medical and psychiatric approach to such patients .
	manualset3
99433	3	400263	5	NULL	NULL	0	NULL	psychiatric illness	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( d ) There is an intimate relationship between unexplained syncope and psychiatric illness , mandating a combined medical and psychiatric approach to such patients .
	manualset3
99434	4	400263	5	NULL	NULL	0	NULL	combined medical and psychiatric approach	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( d ) There is an intimate relationship between unexplained syncope and psychiatric illness , mandating a combined medical and psychiatric approach to such patients .
	manualset3
99435	5	400263	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( d ) There is an intimate relationship between unexplained syncope and psychiatric illness , mandating a combined medical and psychiatric approach to such patients .
	manualset3
99436	1	400264	5	NULL	NULL	0	NULL	group B	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In group B , 83.3 % of patients showed 10 % or more increase in the posttreatment score in comparison with 57.1 % in group A. Improvement was more marked in paucibacillary cases and when the duration of nerve involvement was less than 3 months .
	manualset3
99437	2	400264	5	NULL	NULL	0	NULL	83.3 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In group B , 83.3 % of patients showed 10 % or more increase in the posttreatment score in comparison with 57.1 % in group A. Improvement was more marked in paucibacillary cases and when the duration of nerve involvement was less than 3 months .
	manualset3
99438	3	400264	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In group B , 83.3 % of patients showed 10 % or more increase in the posttreatment score in comparison with 57.1 % in group A. Improvement was more marked in paucibacillary cases and when the duration of nerve involvement was less than 3 months .
	manualset3
99439	4	400264	5	NULL	NULL	0	NULL	10 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In group B , 83.3 % of patients showed 10 % or more increase in the posttreatment score in comparison with 57.1 % in group A. Improvement was more marked in paucibacillary cases and when the duration of nerve involvement was less than 3 months .
	manualset3
99440	5	400264	5	NULL	NULL	NULL	NULL	posttreatment score	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In group B , 83.3 % of patients showed 10 % or more increase in the posttreatment score in comparison with 57.1 % in group A. Improvement was more marked in paucibacillary cases and when the duration of nerve involvement was less than 3 months .
	manualset3
99441	6	400264	5	NULL	NULL	0	NULL	57.1 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In group B , 83.3 % of patients showed 10 % or more increase in the posttreatment score in comparison with 57.1 % in group A. Improvement was more marked in paucibacillary cases and when the duration of nerve involvement was less than 3 months .
	manualset3
99442	7	400264	5	NULL	NULL	0	NULL	group A	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In group B , 83.3 % of patients showed 10 % or more increase in the posttreatment score in comparison with 57.1 % in group A. Improvement was more marked in paucibacillary cases and when the duration of nerve involvement was less than 3 months .
	manualset3
99443	8	400264	5	NULL	NULL	0	NULL	Improvement 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In group B , 83.3 % of patients showed 10 % or more increase in the posttreatment score in comparison with 57.1 % in group A. Improvement was more marked in paucibacillary cases and when the duration of nerve involvement was less than 3 months .
	manualset3
99444	9	400264	5	NULL	NULL	0	NULL	paucibacillary cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In group B , 83.3 % of patients showed 10 % or more increase in the posttreatment score in comparison with 57.1 % in group A. Improvement was more marked in paucibacillary cases and when the duration of nerve involvement was less than 3 months .
	manualset3
99445	10	400264	5	NULL	NULL	0	NULL	duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In group B , 83.3 % of patients showed 10 % or more increase in the posttreatment score in comparison with 57.1 % in group A. Improvement was more marked in paucibacillary cases and when the duration of nerve involvement was less than 3 months .
	manualset3
99446	11	400264	5	NULL	NULL	0	NULL	nerve involvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In group B , 83.3 % of patients showed 10 % or more increase in the posttreatment score in comparison with 57.1 % in group A. Improvement was more marked in paucibacillary cases and when the duration of nerve involvement was less than 3 months .
	manualset3
99447	12	400264	5	NULL	NULL	0	NULL	less than 3 months 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In group B , 83.3 % of patients showed 10 % or more increase in the posttreatment score in comparison with 57.1 % in group A. Improvement was more marked in paucibacillary cases and when the duration of nerve involvement was less than 3 months .
	manualset3
99454	1	400265	5	NULL	NULL	0	NULL	group III	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In group III ( n = 5 ) , a single intravenous bolus injection of 0.8 mg/kg of the F ( ab ' ) 2 fragment of a murine monoclonal antibody ( 7E3 ) against the human platelet GPIIb/IIIa receptor ( 7E3-F ( ab ' ) 2 ) produced stable reperfusion in two of the five dogs , whereas occlusion persisted in the other three .
	manualset3
99455	2	400265	5	NULL	NULL	0	NULL	n = 5	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In group III ( n = 5 ) , a single intravenous bolus injection of 0.8 mg/kg of the F ( ab ' ) 2 fragment of a murine monoclonal antibody ( 7E3 ) against the human platelet GPIIb/IIIa receptor ( 7E3-F ( ab ' ) 2 ) produced stable reperfusion in two of the five dogs , whereas occlusion persisted in the other three .
	manualset3
99456	3	400265	5	NULL	NULL	0	NULL	 single intravenous bolus injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In group III ( n = 5 ) , a single intravenous bolus injection of 0.8 mg/kg of the F ( ab ' ) 2 fragment of a murine monoclonal antibody ( 7E3 ) against the human platelet GPIIb/IIIa receptor ( 7E3-F ( ab ' ) 2 ) produced stable reperfusion in two of the five dogs , whereas occlusion persisted in the other three .
	manualset3
99457	4	400265	5	NULL	NULL	0	NULL	0.8 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In group III ( n = 5 ) , a single intravenous bolus injection of 0.8 mg/kg of the F ( ab ' ) 2 fragment of a murine monoclonal antibody ( 7E3 ) against the human platelet GPIIb/IIIa receptor ( 7E3-F ( ab ' ) 2 ) produced stable reperfusion in two of the five dogs , whereas occlusion persisted in the other three .
	manualset3
99663	5	400265	5	NULL	NULL	0	NULL	F ( ab ' ) 2 fragment of a murine monoclonal antibody ( 7E3 ) against the human platelet GPIIb/IIIa receptor ( 7E3-F ( ab ' ) 2 )	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In group III ( n = 5 ) , a single intravenous bolus injection of 0.8 mg/kg of the F ( ab ' ) 2 fragment of a murine monoclonal antibody ( 7E3 ) against the human platelet GPIIb/IIIa receptor ( 7E3-F ( ab ' ) 2 ) produced stable reperfusion in two of the five dogs , whereas occlusion persisted in the other three .
	manualset3
99664	6	400265	5	NULL	NULL	NULL	NULL	stable reperfusion	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In group III ( n = 5 ) , a single intravenous bolus injection of 0.8 mg/kg of the F ( ab ' ) 2 fragment of a murine monoclonal antibody ( 7E3 ) against the human platelet GPIIb/IIIa receptor ( 7E3-F ( ab ' ) 2 ) produced stable reperfusion in two of the five dogs , whereas occlusion persisted in the other three .
	manualset3
99666	7	400265	5	NULL	NULL	NULL	NULL	two of the five dogs	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In group III ( n = 5 ) , a single intravenous bolus injection of 0.8 mg/kg of the F ( ab ' ) 2 fragment of a murine monoclonal antibody ( 7E3 ) against the human platelet GPIIb/IIIa receptor ( 7E3-F ( ab ' ) 2 ) produced stable reperfusion in two of the five dogs , whereas occlusion persisted in the other three .
	manualset3
99668	8	400265	5	NULL	NULL	0	NULL	occlusion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In group III ( n = 5 ) , a single intravenous bolus injection of 0.8 mg/kg of the F ( ab ' ) 2 fragment of a murine monoclonal antibody ( 7E3 ) against the human platelet GPIIb/IIIa receptor ( 7E3-F ( ab ' ) 2 ) produced stable reperfusion in two of the five dogs , whereas occlusion persisted in the other three .
	manualset3
109512	9	400265	5	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In group III ( n = 5 ) , a single intravenous bolus injection of 0.8 mg/kg of the F ( ab ' ) 2 fragment of a murine monoclonal antibody ( 7E3 ) against the human platelet GPIIb/IIIa receptor ( 7E3-F ( ab ' ) 2 ) produced stable reperfusion in two of the five dogs , whereas occlusion persisted in the other three .
	manualset3
99670	1	400266	5	NULL	NULL	0	NULL	growth chambers	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In growth chambers , the breeding lines N220-1-92 , N222-1-91 , and N320-2-91 were resistant to Meloidoglyne incognita race 3 ; multiplication factors were & lt ; / = 1.0 at both 6 weeks and 10 weeks after inoculation compared with 25.8 and 26.5 for Deltapine 16 at 6 and 10 weeks after inoculation , respectively , and 9.1 and 2.6 for Stoneville 453 .
	manualset3
99689	2	400266	5	NULL	NULL	0	NULL	breeding lines N220-1-92	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In growth chambers , the breeding lines N220-1-92 , N222-1-91 , and N320-2-91 were resistant to Meloidoglyne incognita race 3 ; multiplication factors were & lt ; / = 1.0 at both 6 weeks and 10 weeks after inoculation compared with 25.8 and 26.5 for Deltapine 16 at 6 and 10 weeks after inoculation , respectively , and 9.1 and 2.6 for Stoneville 453 .
	manualset3
99690	3	400266	5	NULL	NULL	0	NULL	breeding lines N222-1-91	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In growth chambers , the breeding lines N220-1-92 , N222-1-91 , and N320-2-91 were resistant to Meloidoglyne incognita race 3 ; multiplication factors were & lt ; / = 1.0 at both 6 weeks and 10 weeks after inoculation compared with 25.8 and 26.5 for Deltapine 16 at 6 and 10 weeks after inoculation , respectively , and 9.1 and 2.6 for Stoneville 453 .
	manualset3
99691	4	400266	5	NULL	NULL	0	NULL	breeding lines N320-2-91	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In growth chambers , the breeding lines N220-1-92 , N222-1-91 , and N320-2-91 were resistant to Meloidoglyne incognita race 3 ; multiplication factors were & lt ; / = 1.0 at both 6 weeks and 10 weeks after inoculation compared with 25.8 and 26.5 for Deltapine 16 at 6 and 10 weeks after inoculation , respectively , and 9.1 and 2.6 for Stoneville 453 .
	manualset3
99692	5	400266	5	NULL	NULL	0	NULL	Meloidoglyne incognita race 3 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In growth chambers , the breeding lines N220-1-92 , N222-1-91 , and N320-2-91 were resistant to Meloidoglyne incognita race 3 ; multiplication factors were & lt ; / = 1.0 at both 6 weeks and 10 weeks after inoculation compared with 25.8 and 26.5 for Deltapine 16 at 6 and 10 weeks after inoculation , respectively , and 9.1 and 2.6 for Stoneville 453 .
	manualset3
99693	6	400266	5	NULL	NULL	0	NULL	lt ; / = 1.0	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In growth chambers , the breeding lines N220-1-92 , N222-1-91 , and N320-2-91 were resistant to Meloidoglyne incognita race 3 ; multiplication factors were & lt ; / = 1.0 at both 6 weeks and 10 weeks after inoculation compared with 25.8 and 26.5 for Deltapine 16 at 6 and 10 weeks after inoculation , respectively , and 9.1 and 2.6 for Stoneville 453 .
	manualset3
99694	7	400266	5	NULL	NULL	NULL	NULL	6 weeks after inoculation	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In growth chambers , the breeding lines N220-1-92 , N222-1-91 , and N320-2-91 were resistant to Meloidoglyne incognita race 3 ; multiplication factors were & lt ; / = 1.0 at both 6 weeks and 10 weeks after inoculation compared with 25.8 and 26.5 for Deltapine 16 at 6 and 10 weeks after inoculation , respectively , and 9.1 and 2.6 for Stoneville 453 .
	manualset3
99695	8	400266	5	NULL	NULL	0	NULL	10 weeks after inoculation	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In growth chambers , the breeding lines N220-1-92 , N222-1-91 , and N320-2-91 were resistant to Meloidoglyne incognita race 3 ; multiplication factors were & lt ; / = 1.0 at both 6 weeks and 10 weeks after inoculation compared with 25.8 and 26.5 for Deltapine 16 at 6 and 10 weeks after inoculation , respectively , and 9.1 and 2.6 for Stoneville 453 .
	manualset3
99696	9	400266	5	NULL	NULL	0	NULL	25.8 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In growth chambers , the breeding lines N220-1-92 , N222-1-91 , and N320-2-91 were resistant to Meloidoglyne incognita race 3 ; multiplication factors were & lt ; / = 1.0 at both 6 weeks and 10 weeks after inoculation compared with 25.8 and 26.5 for Deltapine 16 at 6 and 10 weeks after inoculation , respectively , and 9.1 and 2.6 for Stoneville 453 .
	manualset3
99697	10	400266	5	NULL	NULL	0	NULL	26.5	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In growth chambers , the breeding lines N220-1-92 , N222-1-91 , and N320-2-91 were resistant to Meloidoglyne incognita race 3 ; multiplication factors were & lt ; / = 1.0 at both 6 weeks and 10 weeks after inoculation compared with 25.8 and 26.5 for Deltapine 16 at 6 and 10 weeks after inoculation , respectively , and 9.1 and 2.6 for Stoneville 453 .
	manualset3
99698	11	400266	5	NULL	NULL	0	NULL	Deltapine 16	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In growth chambers , the breeding lines N220-1-92 , N222-1-91 , and N320-2-91 were resistant to Meloidoglyne incognita race 3 ; multiplication factors were & lt ; / = 1.0 at both 6 weeks and 10 weeks after inoculation compared with 25.8 and 26.5 for Deltapine 16 at 6 and 10 weeks after inoculation , respectively , and 9.1 and 2.6 for Stoneville 453 .
	manualset3
99700	12	400266	5	NULL	NULL	0	NULL	6 weeks after inoculation	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In growth chambers , the breeding lines N220-1-92 , N222-1-91 , and N320-2-91 were resistant to Meloidoglyne incognita race 3 ; multiplication factors were & lt ; / = 1.0 at both 6 weeks and 10 weeks after inoculation compared with 25.8 and 26.5 for Deltapine 16 at 6 and 10 weeks after inoculation , respectively , and 9.1 and 2.6 for Stoneville 453 .
	manualset3
99701	13	400266	5	NULL	NULL	0	NULL	10 weeks after inoculation	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In growth chambers , the breeding lines N220-1-92 , N222-1-91 , and N320-2-91 were resistant to Meloidoglyne incognita race 3 ; multiplication factors were & lt ; / = 1.0 at both 6 weeks and 10 weeks after inoculation compared with 25.8 and 26.5 for Deltapine 16 at 6 and 10 weeks after inoculation , respectively , and 9.1 and 2.6 for Stoneville 453 .
	manualset3
99703	14	400266	5	NULL	NULL	0	NULL	9.1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In growth chambers , the breeding lines N220-1-92 , N222-1-91 , and N320-2-91 were resistant to Meloidoglyne incognita race 3 ; multiplication factors were & lt ; / = 1.0 at both 6 weeks and 10 weeks after inoculation compared with 25.8 and 26.5 for Deltapine 16 at 6 and 10 weeks after inoculation , respectively , and 9.1 and 2.6 for Stoneville 453 .
	manualset3
99704	15	400266	5	NULL	NULL	0	NULL	2.6	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In growth chambers , the breeding lines N220-1-92 , N222-1-91 , and N320-2-91 were resistant to Meloidoglyne incognita race 3 ; multiplication factors were & lt ; / = 1.0 at both 6 weeks and 10 weeks after inoculation compared with 25.8 and 26.5 for Deltapine 16 at 6 and 10 weeks after inoculation , respectively , and 9.1 and 2.6 for Stoneville 453 .
	manualset3
99708	16	400266	5	NULL	NULL	0	NULL	Stoneville 453	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In growth chambers , the breeding lines N220-1-92 , N222-1-91 , and N320-2-91 were resistant to Meloidoglyne incognita race 3 ; multiplication factors were & lt ; / = 1.0 at both 6 weeks and 10 weeks after inoculation compared with 25.8 and 26.5 for Deltapine 16 at 6 and 10 weeks after inoculation , respectively , and 9.1 and 2.6 for Stoneville 453 .
	manualset3
99709	17	400266	5	NULL	NULL	0	NULL	multiplication factors	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In growth chambers , the breeding lines N220-1-92 , N222-1-91 , and N320-2-91 were resistant to Meloidoglyne incognita race 3 ; multiplication factors were & lt ; / = 1.0 at both 6 weeks and 10 weeks after inoculation compared with 25.8 and 26.5 for Deltapine 16 at 6 and 10 weeks after inoculation , respectively , and 9.1 and 2.6 for Stoneville 453 .
	manualset3
99711	1	400267	5	NULL	NULL	0	NULL	healthy volunteers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In healthy volunteers , an overall good agreement ( mean ICC : 0.75 and 0.63 for systole and diastole ) was found between the different methods .
	manualset3
99712	2	400267	5	NULL	NULL	0	NULL	overall good agreement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In healthy volunteers , an overall good agreement ( mean ICC : 0.75 and 0.63 for systole and diastole ) was found between the different methods .
	manualset3
99713	3	400267	5	NULL	NULL	0	NULL	mean ICC	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In healthy volunteers , an overall good agreement ( mean ICC : 0.75 and 0.63 for systole and diastole ) was found between the different methods .
	manualset3
99715	4	400267	5	NULL	NULL	0	NULL	0.75	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In healthy volunteers , an overall good agreement ( mean ICC : 0.75 and 0.63 for systole and diastole ) was found between the different methods .
	manualset3
99717	5	400267	5	NULL	NULL	0	NULL	0.63	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In healthy volunteers , an overall good agreement ( mean ICC : 0.75 and 0.63 for systole and diastole ) was found between the different methods .
	manualset3
99718	6	400267	5	NULL	NULL	0	NULL	systole	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In healthy volunteers , an overall good agreement ( mean ICC : 0.75 and 0.63 for systole and diastole ) was found between the different methods .
	manualset3
99719	7	400267	5	NULL	NULL	0	NULL	diastole	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In healthy volunteers , an overall good agreement ( mean ICC : 0.75 and 0.63 for systole and diastole ) was found between the different methods .
	manualset3
99721	8	400267	5	NULL	NULL	NULL	NULL	different methods	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In healthy volunteers , an overall good agreement ( mean ICC : 0.75 and 0.63 for systole and diastole ) was found between the different methods .
	manualset3
99733	1	400268	5	NULL	NULL	0	NULL	hearts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In hearts subjected to severe ischemia , the ratios of AMP : ATP and Cr : PCr were significantly elevated as compared with aerobic hearts .
	manualset3
99738	2	400268	5	NULL	NULL	0	NULL	severe ischemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In hearts subjected to severe ischemia , the ratios of AMP : ATP and Cr : PCr were significantly elevated as compared with aerobic hearts .
	manualset3
99739	3	400268	5	NULL	NULL	NULL	NULL	ratios of AMP : ATP	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In hearts subjected to severe ischemia , the ratios of AMP : ATP and Cr : PCr were significantly elevated as compared with aerobic hearts .
	manualset3
99740	4	400268	5	NULL	NULL	0	NULL	AMP : ATP 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In hearts subjected to severe ischemia , the ratios of AMP : ATP and Cr : PCr were significantly elevated as compared with aerobic hearts .
	manualset3
99743	5	400268	5	NULL	NULL	0	NULL	ratios of Cr : PCr	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In hearts subjected to severe ischemia , the ratios of AMP : ATP and Cr : PCr were significantly elevated as compared with aerobic hearts .
	manualset3
99745	6	400268	5	NULL	NULL	0	NULL	aerobic hearts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In hearts subjected to severe ischemia , the ratios of AMP : ATP and Cr : PCr were significantly elevated as compared with aerobic hearts .
	manualset3
99760	1	400269	5	NULL	NULL	0	NULL	one of 4 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In hematological ones , one of 4 cases with virus associated hemophagocytic syndrome ( VAHS ) took fatal courses in the phase I , others had recovered by early diagnosis and adequate therapies ( pulse therapy of steroids , exchange transfusion etc. ) .
	manualset3
99761	2	400269	5	NULL	NULL	NULL	NULL	virus associated hemophagocytic syndrome ( VAHS )	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In hematological ones , one of 4 cases with virus associated hemophagocytic syndrome ( VAHS ) took fatal courses in the phase I , others had recovered by early diagnosis and adequate therapies ( pulse therapy of steroids , exchange transfusion etc. ) .
	manualset3
99762	3	400269	5	NULL	NULL	0	NULL	fatal courses	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In hematological ones , one of 4 cases with virus associated hemophagocytic syndrome ( VAHS ) took fatal courses in the phase I , others had recovered by early diagnosis and adequate therapies ( pulse therapy of steroids , exchange transfusion etc. ) .
	manualset3
99763	4	400269	5	NULL	NULL	0	NULL	phase I	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In hematological ones , one of 4 cases with virus associated hemophagocytic syndrome ( VAHS ) took fatal courses in the phase I , others had recovered by early diagnosis and adequate therapies ( pulse therapy of steroids , exchange transfusion etc. ) .
	manualset3
99764	5	400269	5	NULL	NULL	0	NULL	early diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In hematological ones , one of 4 cases with virus associated hemophagocytic syndrome ( VAHS ) took fatal courses in the phase I , others had recovered by early diagnosis and adequate therapies ( pulse therapy of steroids , exchange transfusion etc. ) .
	manualset3
99765	6	400269	5	NULL	NULL	0	NULL	adequate therapies 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In hematological ones , one of 4 cases with virus associated hemophagocytic syndrome ( VAHS ) took fatal courses in the phase I , others had recovered by early diagnosis and adequate therapies ( pulse therapy of steroids , exchange transfusion etc. ) .
	manualset3
99766	7	400269	5	NULL	NULL	0	NULL	pulse therapy of steroids	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In hematological ones , one of 4 cases with virus associated hemophagocytic syndrome ( VAHS ) took fatal courses in the phase I , others had recovered by early diagnosis and adequate therapies ( pulse therapy of steroids , exchange transfusion etc. ) .
	manualset3
99767	8	400269	5	NULL	NULL	0	NULL	exchange transfusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In hematological ones , one of 4 cases with virus associated hemophagocytic syndrome ( VAHS ) took fatal courses in the phase I , others had recovered by early diagnosis and adequate therapies ( pulse therapy of steroids , exchange transfusion etc. ) .
	manualset3
99768	1	400270	5	NULL	NULL	NULL	NULL	hormone-supplemented serum-free medium 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In hormone-supplemented serum-free medium , insulin does not stimulate growth of the melanoma cells , while it does stimulate growth of th fibroblast X melanoma hybrid .
	manualset3
99769	2	400270	5	NULL	NULL	0	NULL	insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In hormone-supplemented serum-free medium , insulin does not stimulate growth of the melanoma cells , while it does stimulate growth of th fibroblast X melanoma hybrid .
	manualset3
99770	3	400270	5	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In hormone-supplemented serum-free medium , insulin does not stimulate growth of the melanoma cells , while it does stimulate growth of th fibroblast X melanoma hybrid .
	manualset3
99771	4	400270	5	NULL	NULL	0	NULL	melanoma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In hormone-supplemented serum-free medium , insulin does not stimulate growth of the melanoma cells , while it does stimulate growth of th fibroblast X melanoma hybrid .
	manualset3
99772	5	400270	5	NULL	NULL	0	NULL	growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In hormone-supplemented serum-free medium , insulin does not stimulate growth of the melanoma cells , while it does stimulate growth of th fibroblast X melanoma hybrid .
	manualset3
99773	6	400270	5	NULL	NULL	0	NULL	fibroblast X melanoma hybrid	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In hormone-supplemented serum-free medium , insulin does not stimulate growth of the melanoma cells , while it does stimulate growth of th fibroblast X melanoma hybrid .
	manualset3
99774	1	400271	5	NULL	NULL	0	NULL	human epidermal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In human epidermal cells , previous studies have evidenced that proteasome function is decreased during aging as well as upon UV irradiation , which is the main component of photoaging .
	manualset3
99775	2	400271	5	NULL	NULL	0	NULL	previous studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In human epidermal cells , previous studies have evidenced that proteasome function is decreased during aging as well as upon UV irradiation , which is the main component of photoaging .
	manualset3
99776	3	400271	5	NULL	NULL	0	NULL	proteasome function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In human epidermal cells , previous studies have evidenced that proteasome function is decreased during aging as well as upon UV irradiation , which is the main component of photoaging .
	manualset3
99777	4	400271	5	NULL	NULL	0	NULL	aging	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In human epidermal cells , previous studies have evidenced that proteasome function is decreased during aging as well as upon UV irradiation , which is the main component of photoaging .
	manualset3
99778	5	400271	5	NULL	NULL	0	NULL	UV irradiation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In human epidermal cells , previous studies have evidenced that proteasome function is decreased during aging as well as upon UV irradiation , which is the main component of photoaging .
	manualset3
99781	6	400271	5	NULL	NULL	0	NULL	main component	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In human epidermal cells , previous studies have evidenced that proteasome function is decreased during aging as well as upon UV irradiation , which is the main component of photoaging .
	manualset3
99782	7	400271	5	NULL	NULL	0	NULL	photoaging	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In human epidermal cells , previous studies have evidenced that proteasome function is decreased during aging as well as upon UV irradiation , which is the main component of photoaging .
	manualset3
99810	1	400272	5	NULL	NULL	0	NULL	X = H	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	( formula ; see text ) where : X = H , CH3 R = H , 2-F , 3-F , 4-F , 3-Cl , 4-Cl R ' = H , 4-F , 4-Cl These compounds were prepared by the general synthetic procedure previously reported for the 1 , 3-thiazolidin-4-one derivatives already prepared and screened in this SARs program .
	manualset3
99811	2	400272	5	NULL	NULL	0	NULL	CH3 R = H	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( formula ; see text ) where : X = H , CH3 R = H , 2-F , 3-F , 4-F , 3-Cl , 4-Cl R ' = H , 4-F , 4-Cl These compounds were prepared by the general synthetic procedure previously reported for the 1 , 3-thiazolidin-4-one derivatives already prepared and screened in this SARs program .
	manualset3
99812	3	400272	5	NULL	NULL	0	NULL	2-F , 3-F , 4-F , 3-Cl , 4-Cl R ' = H	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	( formula ; see text ) where : X = H , CH3 R = H , 2-F , 3-F , 4-F , 3-Cl , 4-Cl R ' = H , 4-F , 4-Cl These compounds were prepared by the general synthetic procedure previously reported for the 1 , 3-thiazolidin-4-one derivatives already prepared and screened in this SARs program .
	manualset3
99813	4	400272	5	NULL	NULL	0	NULL	4-F	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	( formula ; see text ) where : X = H , CH3 R = H , 2-F , 3-F , 4-F , 3-Cl , 4-Cl R ' = H , 4-F , 4-Cl These compounds were prepared by the general synthetic procedure previously reported for the 1 , 3-thiazolidin-4-one derivatives already prepared and screened in this SARs program .
	manualset3
99814	5	400272	5	NULL	NULL	0	NULL	4-Cl	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	( formula ; see text ) where : X = H , CH3 R = H , 2-F , 3-F , 4-F , 3-Cl , 4-Cl R ' = H , 4-F , 4-Cl These compounds were prepared by the general synthetic procedure previously reported for the 1 , 3-thiazolidin-4-one derivatives already prepared and screened in this SARs program .
	manualset3
99815	6	400272	5	NULL	NULL	0	NULL	compounds 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( formula ; see text ) where : X = H , CH3 R = H , 2-F , 3-F , 4-F , 3-Cl , 4-Cl R ' = H , 4-F , 4-Cl These compounds were prepared by the general synthetic procedure previously reported for the 1 , 3-thiazolidin-4-one derivatives already prepared and screened in this SARs program .
	manualset3
99816	7	400272	5	NULL	NULL	0	NULL	general synthetic procedure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( formula ; see text ) where : X = H , CH3 R = H , 2-F , 3-F , 4-F , 3-Cl , 4-Cl R ' = H , 4-F , 4-Cl These compounds were prepared by the general synthetic procedure previously reported for the 1 , 3-thiazolidin-4-one derivatives already prepared and screened in this SARs program .
	manualset3
99817	8	400272	5	NULL	NULL	0	NULL	1 , 3-thiazolidin-4-one derivatives	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( formula ; see text ) where : X = H , CH3 R = H , 2-F , 3-F , 4-F , 3-Cl , 4-Cl R ' = H , 4-F , 4-Cl These compounds were prepared by the general synthetic procedure previously reported for the 1 , 3-thiazolidin-4-one derivatives already prepared and screened in this SARs program .
	manualset3
99821	9	400272	5	NULL	NULL	0	NULL	SARs program	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( formula ; see text ) where : X = H , CH3 R = H , 2-F , 3-F , 4-F , 3-Cl , 4-Cl R ' = H , 4-F , 4-Cl These compounds were prepared by the general synthetic procedure previously reported for the 1 , 3-thiazolidin-4-one derivatives already prepared and screened in this SARs program .
	manualset3
99822	1	400273	5	NULL	NULL	0	NULL	human lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In human lymphocytes no significant changes were observed in either MI or SCE .
	manualset3
99823	2	400273	5	NULL	NULL	0	NULL	MI	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In human lymphocytes no significant changes were observed in either MI or SCE .
	manualset3
99824	3	400273	5	NULL	NULL	0	NULL	SCE	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In human lymphocytes no significant changes were observed in either MI or SCE .
	manualset3
99826	1	400274	5	NULL	NULL	0	NULL	humans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In humans acute intravenous infusions of carbohydrates do not appear to affect either protein degradation or leucine oxidation .
	manualset3
99827	2	400274	5	NULL	NULL	0	NULL	acute intravenous infusions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In humans acute intravenous infusions of carbohydrates do not appear to affect either protein degradation or leucine oxidation .
	manualset3
99828	3	400274	5	NULL	NULL	0	NULL	carbohydrates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In humans acute intravenous infusions of carbohydrates do not appear to affect either protein degradation or leucine oxidation .
	manualset3
99829	4	400274	5	NULL	NULL	0	NULL	protein degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In humans acute intravenous infusions of carbohydrates do not appear to affect either protein degradation or leucine oxidation .
	manualset3
99830	5	400274	5	NULL	NULL	0	NULL	leucine oxidation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In humans acute intravenous infusions of carbohydrates do not appear to affect either protein degradation or leucine oxidation .
	manualset3
99831	1	400275	5	NULL	NULL	0	NULL	ifn ( - / - ) mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In ifn ( - / - ) mice , a marked increase in cellular infiltrates and chronic pathology was associated with an increased Th17 response .
	manualset3
99840	2	400275	5	NULL	NULL	0	NULL	cellular infiltrates	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In ifn ( - / - ) mice , a marked increase in cellular infiltrates and chronic pathology was associated with an increased Th17 response .
	manualset3
99841	3	400275	5	NULL	NULL	NULL	NULL	chronic pathology	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In ifn ( - / - ) mice , a marked increase in cellular infiltrates and chronic pathology was associated with an increased Th17 response .
	manualset3
99842	4	400275	5	NULL	NULL	0	NULL	Th17 response 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In ifn ( - / - ) mice , a marked increase in cellular infiltrates and chronic pathology was associated with an increased Th17 response .
	manualset3
99843	1	400276	5	NULL	NULL	0	NULL	immunoblotting	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In immunoblotting it was shown that the molecule in human milk exclusively stained with III D 5 also binds peanut agglutinin ( PNA ) and Ricinus communis .
	manualset3
99844	2	400276	5	NULL	NULL	0	NULL	molecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In immunoblotting it was shown that the molecule in human milk exclusively stained with III D 5 also binds peanut agglutinin ( PNA ) and Ricinus communis .
	manualset3
99845	3	400276	5	NULL	NULL	0	NULL	human milk	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	In immunoblotting it was shown that the molecule in human milk exclusively stained with III D 5 also binds peanut agglutinin ( PNA ) and Ricinus communis .
	manualset3
99928	4	400276	5	NULL	NULL	0	NULL	III D 5	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In immunoblotting it was shown that the molecule in human milk exclusively stained with III D 5 also binds peanut agglutinin ( PNA ) and Ricinus communis .
	manualset3
99929	5	400276	5	NULL	NULL	0	NULL	peanut agglutinin ( PNA )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In immunoblotting it was shown that the molecule in human milk exclusively stained with III D 5 also binds peanut agglutinin ( PNA ) and Ricinus communis .
	manualset3
99930	6	400276	5	NULL	NULL	0	NULL	Ricinus communis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In immunoblotting it was shown that the molecule in human milk exclusively stained with III D 5 also binds peanut agglutinin ( PNA ) and Ricinus communis .
	manualset3
99931	1	400277	5	NULL	NULL	0	NULL	indolent NHL	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In indolent NHL , rituximab has shown useful response rates , both as first-line therapy in relapsed disease .
	manualset3
99932	2	400277	5	NULL	NULL	0	NULL	rituximab	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In indolent NHL , rituximab has shown useful response rates , both as first-line therapy in relapsed disease .
	manualset3
99933	3	400277	5	NULL	NULL	0	NULL	response rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In indolent NHL , rituximab has shown useful response rates , both as first-line therapy in relapsed disease .
	manualset3
99934	4	400277	5	NULL	NULL	0	NULL	first-line therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In indolent NHL , rituximab has shown useful response rates , both as first-line therapy in relapsed disease .
	manualset3
99935	5	400277	5	NULL	NULL	0	NULL	relapsed disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In indolent NHL , rituximab has shown useful response rates , both as first-line therapy in relapsed disease .
	manualset3
99936	1	400278	5	NULL	NULL	0	NULL	inhomogeneous fibers	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In inhomogeneous fibers with adjacent well-coupled and poorly coupled regions , increasing rho ( oeff ) in the poorly coupled region also reduces source-load mismatch , which delays the onset of conduction block and reduces the dispersion of repolarization at the transition between the two regions .
	manualset3
99937	2	400278	5	NULL	NULL	0	NULL	well-coupled and poorly coupled regions	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In inhomogeneous fibers with adjacent well-coupled and poorly coupled regions , increasing rho ( oeff ) in the poorly coupled region also reduces source-load mismatch , which delays the onset of conduction block and reduces the dispersion of repolarization at the transition between the two regions .
	manualset3
99938	3	400278	5	NULL	NULL	0	NULL	rho(oeff)	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In inhomogeneous fibers with adjacent well-coupled and poorly coupled regions , increasing rho ( oeff ) in the poorly coupled region also reduces source-load mismatch , which delays the onset of conduction block and reduces the dispersion of repolarization at the transition between the two regions .
	manualset3
99939	4	400278	5	NULL	NULL	0	NULL	poorly coupled region	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In inhomogeneous fibers with adjacent well-coupled and poorly coupled regions , increasing rho ( oeff ) in the poorly coupled region also reduces source-load mismatch , which delays the onset of conduction block and reduces the dispersion of repolarization at the transition between the two regions .
	manualset3
99940	5	400278	5	NULL	NULL	0	NULL	conduction block	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In inhomogeneous fibers with adjacent well-coupled and poorly coupled regions , increasing rho ( oeff ) in the poorly coupled region also reduces source-load mismatch , which delays the onset of conduction block and reduces the dispersion of repolarization at the transition between the two regions .
	manualset3
99941	6	400278	5	NULL	NULL	NULL	NULL	repolarization	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In inhomogeneous fibers with adjacent well-coupled and poorly coupled regions , increasing rho ( oeff ) in the poorly coupled region also reduces source-load mismatch , which delays the onset of conduction block and reduces the dispersion of repolarization at the transition between the two regions .
	manualset3
99942	7	400278	5	NULL	NULL	0	NULL	transition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In inhomogeneous fibers with adjacent well-coupled and poorly coupled regions , increasing rho ( oeff ) in the poorly coupled region also reduces source-load mismatch , which delays the onset of conduction block and reduces the dispersion of repolarization at the transition between the two regions .
	manualset3
99943	8	400278	5	NULL	NULL	NULL	NULL	two regions	AnatomicalPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In inhomogeneous fibers with adjacent well-coupled and poorly coupled regions , increasing rho ( oeff ) in the poorly coupled region also reduces source-load mismatch , which delays the onset of conduction block and reduces the dispersion of repolarization at the transition between the two regions .
	manualset3
109513	9	400278	5	NULL	NULL	0	NULL	onset	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In inhomogeneous fibers with adjacent well-coupled and poorly coupled regions , increasing rho ( oeff ) in the poorly coupled region also reduces source-load mismatch , which delays the onset of conduction block and reduces the dispersion of repolarization at the transition between the two regions .
	manualset3
109514	10	400278	5	NULL	NULL	0	NULL	dispersion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In inhomogeneous fibers with adjacent well-coupled and poorly coupled regions , increasing rho ( oeff ) in the poorly coupled region also reduces source-load mismatch , which delays the onset of conduction block and reduces the dispersion of repolarization at the transition between the two regions .
	manualset3
99944	2	400279	5	NULL	NULL	NULL	NULL	4 weeks-3 years	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( g ) Outcome after 4 weeks-3 years included no or mild neurological deficits in five patients , marked deficits in three , persistent locked-in syndrome in one , and persistent vegetative state in one .
	manualset3
99945	3	400279	5	NULL	NULL	NULL	NULL	no or mild neurological deficits	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( g ) Outcome after 4 weeks-3 years included no or mild neurological deficits in five patients , marked deficits in three , persistent locked-in syndrome in one , and persistent vegetative state in one .
	manualset3
99946	4	400279	5	NULL	NULL	NULL	NULL	five patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( g ) Outcome after 4 weeks-3 years included no or mild neurological deficits in five patients , marked deficits in three , persistent locked-in syndrome in one , and persistent vegetative state in one .
	manualset3
99947	5	400279	5	NULL	NULL	NULL	NULL	deficits	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( g ) Outcome after 4 weeks-3 years included no or mild neurological deficits in five patients , marked deficits in three , persistent locked-in syndrome in one , and persistent vegetative state in one .
	manualset3
99948	7	400279	5	NULL	NULL	NULL	NULL	persistent locked-in syndrome	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( g ) Outcome after 4 weeks-3 years included no or mild neurological deficits in five patients , marked deficits in three , persistent locked-in syndrome in one , and persistent vegetative state in one .
	manualset3
99949	9	400279	5	NULL	NULL	NULL	NULL	persistent vegetative state	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( g ) Outcome after 4 weeks-3 years included no or mild neurological deficits in five patients , marked deficits in three , persistent locked-in syndrome in one , and persistent vegetative state in one .
	manualset3
109515	1	400279	5	NULL	NULL	0	NULL	Outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( g ) Outcome after 4 weeks-3 years included no or mild neurological deficits in five patients , marked deficits in three , persistent locked-in syndrome in one , and persistent vegetative state in one .
	manualset3
109516	6	400279	5	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( g ) Outcome after 4 weeks-3 years included no or mild neurological deficits in five patients , marked deficits in three , persistent locked-in syndrome in one , and persistent vegetative state in one .
	manualset3
109517	8	400279	5	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( g ) Outcome after 4 weeks-3 years included no or mild neurological deficits in five patients , marked deficits in three , persistent locked-in syndrome in one , and persistent vegetative state in one .
	manualset3
109518	10	400279	5	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( g ) Outcome after 4 weeks-3 years included no or mild neurological deficits in five patients , marked deficits in three , persistent locked-in syndrome in one , and persistent vegetative state in one .
	manualset3
99950	1	400280	5	NULL	NULL	0	NULL	large lens capsule tears	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In large lens capsule tears early lens extraction may prevent severe uveitis and may retain functional vision .
	manualset3
99951	2	400280	5	NULL	NULL	0	NULL	early lens extraction	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In large lens capsule tears early lens extraction may prevent severe uveitis and may retain functional vision .
	manualset3
99952	3	400280	5	NULL	NULL	0	NULL	severe uveitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In large lens capsule tears early lens extraction may prevent severe uveitis and may retain functional vision .
	manualset3
99953	4	400280	5	NULL	NULL	0	NULL	functional vision	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In large lens capsule tears early lens extraction may prevent severe uveitis and may retain functional vision .
	manualset3
99954	1	400281	5	NULL	NULL	0	NULL	learning rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In learning rats the specific radioactivity of neuronal DNA was markedly decreased in the hippocampus and remaining brain .
	manualset3
99955	2	400281	5	NULL	NULL	0	NULL	specific radioactivity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In learning rats the specific radioactivity of neuronal DNA was markedly decreased in the hippocampus and remaining brain .
	manualset3
99956	3	400281	5	NULL	NULL	0	NULL	neuronal DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In learning rats the specific radioactivity of neuronal DNA was markedly decreased in the hippocampus and remaining brain .
	manualset3
99957	4	400281	5	NULL	NULL	0	NULL	hippocampus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In learning rats the specific radioactivity of neuronal DNA was markedly decreased in the hippocampus and remaining brain .
	manualset3
99958	5	400281	5	NULL	NULL	0	NULL	remaining brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In learning rats the specific radioactivity of neuronal DNA was markedly decreased in the hippocampus and remaining brain .
	manualset3
99959	1	400282	5	NULL	NULL	0	NULL	lepromatous leprosy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In lepromatous leprosy and rhinoscleroma the helper/inducer T cells and suppressor/cytotoxic T cells were both diffusely distributed among the mononuclear phagocytes ( histiocytes ) without any discernible mantle .
	manualset3
99960	2	400282	5	NULL	NULL	0	NULL	rhinoscleroma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In lepromatous leprosy and rhinoscleroma the helper/inducer T cells and suppressor/cytotoxic T cells were both diffusely distributed among the mononuclear phagocytes ( histiocytes ) without any discernible mantle .
	manualset3
99961	3	400282	5	NULL	NULL	0	NULL	helper/inducer T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In lepromatous leprosy and rhinoscleroma the helper/inducer T cells and suppressor/cytotoxic T cells were both diffusely distributed among the mononuclear phagocytes ( histiocytes ) without any discernible mantle .
	manualset3
99962	4	400282	5	NULL	NULL	0	NULL	suppressor/cytotoxic T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In lepromatous leprosy and rhinoscleroma the helper/inducer T cells and suppressor/cytotoxic T cells were both diffusely distributed among the mononuclear phagocytes ( histiocytes ) without any discernible mantle .
	manualset3
99963	5	400282	5	NULL	NULL	0	NULL	mononuclear phagocytes ( histiocytes )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In lepromatous leprosy and rhinoscleroma the helper/inducer T cells and suppressor/cytotoxic T cells were both diffusely distributed among the mononuclear phagocytes ( histiocytes ) without any discernible mantle .
	manualset3
99964	1	400283	5	NULL	NULL	0	NULL	15 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In less than 15 % of Insp and Pre-I cells and in 20 % of Exp neurons , termination of hyperpolarizing pulses led to low voltage-activated ( LVA ) Ca2 + spikes with a threshold potential of between -70 and -60 mV ( n = 7 ) .
	manualset3
99965	2	400283	5	NULL	NULL	0	NULL	Insp cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In less than 15 % of Insp and Pre-I cells and in 20 % of Exp neurons , termination of hyperpolarizing pulses led to low voltage-activated ( LVA ) Ca2 + spikes with a threshold potential of between -70 and -60 mV ( n = 7 ) .
	manualset3
99966	3	400283	5	NULL	NULL	0	NULL	Pre-I cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In less than 15 % of Insp and Pre-I cells and in 20 % of Exp neurons , termination of hyperpolarizing pulses led to low voltage-activated ( LVA ) Ca2 + spikes with a threshold potential of between -70 and -60 mV ( n = 7 ) .
	manualset3
99967	4	400283	5	NULL	NULL	0	NULL	20 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In less than 15 % of Insp and Pre-I cells and in 20 % of Exp neurons , termination of hyperpolarizing pulses led to low voltage-activated ( LVA ) Ca2 + spikes with a threshold potential of between -70 and -60 mV ( n = 7 ) .
	manualset3
99968	5	400283	5	NULL	NULL	0	NULL	Exp neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In less than 15 % of Insp and Pre-I cells and in 20 % of Exp neurons , termination of hyperpolarizing pulses led to low voltage-activated ( LVA ) Ca2 + spikes with a threshold potential of between -70 and -60 mV ( n = 7 ) .
	manualset3
99969	6	400283	5	NULL	NULL	0	NULL	termination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In less than 15 % of Insp and Pre-I cells and in 20 % of Exp neurons , termination of hyperpolarizing pulses led to low voltage-activated ( LVA ) Ca2 + spikes with a threshold potential of between -70 and -60 mV ( n = 7 ) .
	manualset3
99970	7	400283	5	NULL	NULL	NULL	NULL	hyperpolarizing pulses	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In less than 15 % of Insp and Pre-I cells and in 20 % of Exp neurons , termination of hyperpolarizing pulses led to low voltage-activated ( LVA ) Ca2 + spikes with a threshold potential of between -70 and -60 mV ( n = 7 ) .
	manualset3
99971	8	400283	5	NULL	NULL	0	NULL	low voltage-activated ( LVA ) Ca2 + spikes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In less than 15 % of Insp and Pre-I cells and in 20 % of Exp neurons , termination of hyperpolarizing pulses led to low voltage-activated ( LVA ) Ca2 + spikes with a threshold potential of between -70 and -60 mV ( n = 7 ) .
	manualset3
99972	9	400283	5	NULL	NULL	0	NULL	threshold potential	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In less than 15 % of Insp and Pre-I cells and in 20 % of Exp neurons , termination of hyperpolarizing pulses led to low voltage-activated ( LVA ) Ca2 + spikes with a threshold potential of between -70 and -60 mV ( n = 7 ) .
	manualset3
99973	10	400283	5	NULL	NULL	0	NULL	-70 and -60 mV ( n = 7 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In less than 15 % of Insp and Pre-I cells and in 20 % of Exp neurons , termination of hyperpolarizing pulses led to low voltage-activated ( LVA ) Ca2 + spikes with a threshold potential of between -70 and -60 mV ( n = 7 ) .
	manualset3
99974	1	400284	5	NULL	NULL	0	NULL	leukemia L 5222	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In leukemia L 5222 all nitrosoureas except compounds 7 , 8 , 11 effected cures .
	manualset3
99975	2	400284	5	NULL	NULL	NULL	NULL	nitrosoureas	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In leukemia L 5222 all nitrosoureas except compounds 7 , 8 , 11 effected cures .
	manualset3
99976	3	400284	5	NULL	NULL	NULL	NULL	compound 7	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In leukemia L 5222 all nitrosoureas except compounds 7 , 8 , 11 effected cures .
	manualset3
99977	4	400284	5	NULL	NULL	0	NULL	compounds 8	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In leukemia L 5222 all nitrosoureas except compounds 7 , 8 , 11 effected cures .
	manualset3
99978	5	400284	5	NULL	NULL	0	NULL	compound 11	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In leukemia L 5222 all nitrosoureas except compounds 7 , 8 , 11 effected cures .
	manualset3
99979	1	400285	5	NULL	NULL	0	NULL	ER stress	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In light of this , ER stress has been shown to trigger both apoptosis and autophagy , and act as an important mediator linking the two programmed cell death pathways .
	manualset3
99980	2	400285	5	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In light of this , ER stress has been shown to trigger both apoptosis and autophagy , and act as an important mediator linking the two programmed cell death pathways .
	manualset3
99981	3	400285	5	NULL	NULL	0	NULL	autophagy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In light of this , ER stress has been shown to trigger both apoptosis and autophagy , and act as an important mediator linking the two programmed cell death pathways .
	manualset3
99982	4	400285	5	NULL	NULL	0	NULL	important mediator 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In light of this , ER stress has been shown to trigger both apoptosis and autophagy , and act as an important mediator linking the two programmed cell death pathways .
	manualset3
99983	5	400285	5	NULL	NULL	0	NULL	two programmed cell death pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In light of this , ER stress has been shown to trigger both apoptosis and autophagy , and act as an important mediator linking the two programmed cell death pathways .
	manualset3
99984	1	400286	5	NULL	NULL	0	NULL	 liver-specific FoxO knock-out mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In liver-specific FoxO knock-out mice , SREBP-1c expression was increased 2-fold .
	manualset3
99985	2	400286	5	NULL	NULL	0	NULL	SREBP-1c expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In liver-specific FoxO knock-out mice , SREBP-1c expression was increased 2-fold .
	manualset3
109519	3	400286	5	NULL	NULL	0	NULL	2-fold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In liver-specific FoxO knock-out mice , SREBP-1c expression was increased 2-fold .
	manualset3
99986	1	400287	5	NULL	NULL	0	NULL	 lymphoid cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In lymphoid cells of all the patients studied ( except of ALL ) the glycosidases activity was decreased as compared with that of normal mononuclear cells and immature myeloid cells .
	manualset3
99987	2	400287	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In lymphoid cells of all the patients studied ( except of ALL ) the glycosidases activity was decreased as compared with that of normal mononuclear cells and immature myeloid cells .
	manualset3
99988	3	400287	5	NULL	NULL	0	NULL	ALL	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In lymphoid cells of all the patients studied ( except of ALL ) the glycosidases activity was decreased as compared with that of normal mononuclear cells and immature myeloid cells .
	manualset3
99989	4	400287	5	NULL	NULL	0	NULL	glycosidases activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In lymphoid cells of all the patients studied ( except of ALL ) the glycosidases activity was decreased as compared with that of normal mononuclear cells and immature myeloid cells .
	manualset3
99990	5	400287	5	NULL	NULL	0	NULL	normal mononuclear cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In lymphoid cells of all the patients studied ( except of ALL ) the glycosidases activity was decreased as compared with that of normal mononuclear cells and immature myeloid cells .
	manualset3
99991	6	400287	5	NULL	NULL	0	NULL	immature myeloid cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In lymphoid cells of all the patients studied ( except of ALL ) the glycosidases activity was decreased as compared with that of normal mononuclear cells and immature myeloid cells .
	manualset3
99992	1	400288	5	NULL	NULL	0	NULL	maintenance treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In maintenance treatment of GORD , PPIs are the most effective drugs , offering the possibility of keeping nearly all patients in remission with adjusted doses .
	manualset3
99993	2	400288	5	NULL	NULL	0	NULL	GORD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In maintenance treatment of GORD , PPIs are the most effective drugs , offering the possibility of keeping nearly all patients in remission with adjusted doses .
	manualset3
99994	3	400288	5	NULL	NULL	0	NULL	PPIs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In maintenance treatment of GORD , PPIs are the most effective drugs , offering the possibility of keeping nearly all patients in remission with adjusted doses .
	manualset3
99995	4	400288	5	NULL	NULL	0	NULL	most effective drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In maintenance treatment of GORD , PPIs are the most effective drugs , offering the possibility of keeping nearly all patients in remission with adjusted doses .
	manualset3
99996	5	400288	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In maintenance treatment of GORD , PPIs are the most effective drugs , offering the possibility of keeping nearly all patients in remission with adjusted doses .
	manualset3
99997	6	400288	5	NULL	NULL	0	NULL	remission 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In maintenance treatment of GORD , PPIs are the most effective drugs , offering the possibility of keeping nearly all patients in remission with adjusted doses .
	manualset3
99998	7	400288	5	NULL	NULL	0	NULL	adjusted doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In maintenance treatment of GORD , PPIs are the most effective drugs , offering the possibility of keeping nearly all patients in remission with adjusted doses .
	manualset3
99999	1	400289	5	NULL	NULL	0	NULL	many countries 	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In many countries , the male : female ratio at birth has varied significantly over the past century , but the reasons for these changes have been unclear .
	manualset3
100000	2	400289	5	NULL	NULL	0	NULL	male : female ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In many countries , the male : female ratio at birth has varied significantly over the past century , but the reasons for these changes have been unclear .
	manualset3
100001	3	400289	5	NULL	NULL	0	NULL	birth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In many countries , the male : female ratio at birth has varied significantly over the past century , but the reasons for these changes have been unclear .
	manualset3
100002	4	400289	5	NULL	NULL	0	NULL	past century	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In many countries , the male : female ratio at birth has varied significantly over the past century , but the reasons for these changes have been unclear .
	manualset3
100003	1	400290	5	NULL	NULL	0	NULL	higher plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In many higher plants , cellulose synthesis is inhibited by isoxaben and thiazolidinone herbicides such as 5-tert-butyl-carbamoyloxy-3 - ( 3-trifluromethyl ) phenyl-4-thiazolidinone .
	manualset3
100004	2	400290	5	NULL	NULL	0	NULL	cellulose synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In many higher plants , cellulose synthesis is inhibited by isoxaben and thiazolidinone herbicides such as 5-tert-butyl-carbamoyloxy-3 - ( 3-trifluromethyl ) phenyl-4-thiazolidinone .
	manualset3
100005	3	400290	5	NULL	NULL	0	NULL	isoxaben 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In many higher plants , cellulose synthesis is inhibited by isoxaben and thiazolidinone herbicides such as 5-tert-butyl-carbamoyloxy-3 - ( 3-trifluromethyl ) phenyl-4-thiazolidinone .
	manualset3
100006	4	400290	5	NULL	NULL	0	NULL	thiazolidinone herbicides 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In many higher plants , cellulose synthesis is inhibited by isoxaben and thiazolidinone herbicides such as 5-tert-butyl-carbamoyloxy-3 - ( 3-trifluromethyl ) phenyl-4-thiazolidinone .
	manualset3
100007	5	400290	5	NULL	NULL	0	NULL	 5-tert-butyl-carbamoyloxy-3 - ( 3-trifluromethyl ) phenyl-4-thiazolidinone	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In many higher plants , cellulose synthesis is inhibited by isoxaben and thiazolidinone herbicides such as 5-tert-butyl-carbamoyloxy-3 - ( 3-trifluromethyl ) phenyl-4-thiazolidinone .
	manualset3
100008	1	400291	5	NULL	NULL	0	NULL	megatrials 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In megatrials with simvastatin , the overall incidence of myopathy was 0.025 % .
	manualset3
100009	2	400291	5	NULL	NULL	0	NULL	simvastatin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In megatrials with simvastatin , the overall incidence of myopathy was 0.025 % .
	manualset3
100010	3	400291	5	NULL	NULL	0	NULL	overall incidence 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In megatrials with simvastatin , the overall incidence of myopathy was 0.025 % .
	manualset3
100011	4	400291	5	NULL	NULL	0	NULL	myopathy 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In megatrials with simvastatin , the overall incidence of myopathy was 0.025 % .
	manualset3
100012	5	400291	5	NULL	NULL	0	NULL	0.025 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In megatrials with simvastatin , the overall incidence of myopathy was 0.025 % .
	manualset3
100013	1	400292	5	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In men aged 40-59 years , the ranking of increasing cost-effectiveness was : smoking cessation ( $ 2 , 608-3 , 738 per LYG ) ; treatment of moderate and severe hypertension ( $ 8 , 564-38 , 678 per LYG ) ; treatment of mild hypertension ( $ 11 , 906-59 , 840 per LYG ) ; dietary treatment ( $ 16 , 143-20 , 158 per LYG ) ; and drug treatment of hypercholesterolemia ( $ 33 , 850-81 , 010 per LYG ) .
	manualset3
100014	2	400292	5	NULL	NULL	0	NULL	40-59 years	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In men aged 40-59 years , the ranking of increasing cost-effectiveness was : smoking cessation ( $ 2 , 608-3 , 738 per LYG ) ; treatment of moderate and severe hypertension ( $ 8 , 564-38 , 678 per LYG ) ; treatment of mild hypertension ( $ 11 , 906-59 , 840 per LYG ) ; dietary treatment ( $ 16 , 143-20 , 158 per LYG ) ; and drug treatment of hypercholesterolemia ( $ 33 , 850-81 , 010 per LYG ) .
	manualset3
100015	3	400292	5	NULL	NULL	0	NULL	smoking cessation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In men aged 40-59 years , the ranking of increasing cost-effectiveness was : smoking cessation ( $ 2 , 608-3 , 738 per LYG ) ; treatment of moderate and severe hypertension ( $ 8 , 564-38 , 678 per LYG ) ; treatment of mild hypertension ( $ 11 , 906-59 , 840 per LYG ) ; dietary treatment ( $ 16 , 143-20 , 158 per LYG ) ; and drug treatment of hypercholesterolemia ( $ 33 , 850-81 , 010 per LYG ) .
	manualset3
100016	4	400292	5	NULL	NULL	0	NULL	$ 2 , 608-3 , 738 per LYG	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In men aged 40-59 years , the ranking of increasing cost-effectiveness was : smoking cessation ( $ 2 , 608-3 , 738 per LYG ) ; treatment of moderate and severe hypertension ( $ 8 , 564-38 , 678 per LYG ) ; treatment of mild hypertension ( $ 11 , 906-59 , 840 per LYG ) ; dietary treatment ( $ 16 , 143-20 , 158 per LYG ) ; and drug treatment of hypercholesterolemia ( $ 33 , 850-81 , 010 per LYG ) .
	manualset3
100017	5	400292	5	NULL	NULL	NULL	NULL	treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In men aged 40-59 years , the ranking of increasing cost-effectiveness was : smoking cessation ( $ 2 , 608-3 , 738 per LYG ) ; treatment of moderate and severe hypertension ( $ 8 , 564-38 , 678 per LYG ) ; treatment of mild hypertension ( $ 11 , 906-59 , 840 per LYG ) ; dietary treatment ( $ 16 , 143-20 , 158 per LYG ) ; and drug treatment of hypercholesterolemia ( $ 33 , 850-81 , 010 per LYG ) .
	manualset3
100018	7	400292	5	NULL	NULL	NULL	NULL	severe hypertension	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In men aged 40-59 years , the ranking of increasing cost-effectiveness was : smoking cessation ( $ 2 , 608-3 , 738 per LYG ) ; treatment of moderate and severe hypertension ( $ 8 , 564-38 , 678 per LYG ) ; treatment of mild hypertension ( $ 11 , 906-59 , 840 per LYG ) ; dietary treatment ( $ 16 , 143-20 , 158 per LYG ) ; and drug treatment of hypercholesterolemia ( $ 33 , 850-81 , 010 per LYG ) .
	manualset3
100019	8	400292	5	NULL	NULL	NULL	NULL	$ 8 , 564-38 , 678 per LYG	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In men aged 40-59 years , the ranking of increasing cost-effectiveness was : smoking cessation ( $ 2 , 608-3 , 738 per LYG ) ; treatment of moderate and severe hypertension ( $ 8 , 564-38 , 678 per LYG ) ; treatment of mild hypertension ( $ 11 , 906-59 , 840 per LYG ) ; dietary treatment ( $ 16 , 143-20 , 158 per LYG ) ; and drug treatment of hypercholesterolemia ( $ 33 , 850-81 , 010 per LYG ) .
	manualset3
100020	6	400292	5	NULL	NULL	0	NULL	moderate hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In men aged 40-59 years , the ranking of increasing cost-effectiveness was : smoking cessation ( $ 2 , 608-3 , 738 per LYG ) ; treatment of moderate and severe hypertension ( $ 8 , 564-38 , 678 per LYG ) ; treatment of mild hypertension ( $ 11 , 906-59 , 840 per LYG ) ; dietary treatment ( $ 16 , 143-20 , 158 per LYG ) ; and drug treatment of hypercholesterolemia ( $ 33 , 850-81 , 010 per LYG ) .
	manualset3
100021	9	400292	5	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In men aged 40-59 years , the ranking of increasing cost-effectiveness was : smoking cessation ( $ 2 , 608-3 , 738 per LYG ) ; treatment of moderate and severe hypertension ( $ 8 , 564-38 , 678 per LYG ) ; treatment of mild hypertension ( $ 11 , 906-59 , 840 per LYG ) ; dietary treatment ( $ 16 , 143-20 , 158 per LYG ) ; and drug treatment of hypercholesterolemia ( $ 33 , 850-81 , 010 per LYG ) .
	manualset3
100022	10	400292	5	NULL	NULL	0	NULL	mild hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In men aged 40-59 years , the ranking of increasing cost-effectiveness was : smoking cessation ( $ 2 , 608-3 , 738 per LYG ) ; treatment of moderate and severe hypertension ( $ 8 , 564-38 , 678 per LYG ) ; treatment of mild hypertension ( $ 11 , 906-59 , 840 per LYG ) ; dietary treatment ( $ 16 , 143-20 , 158 per LYG ) ; and drug treatment of hypercholesterolemia ( $ 33 , 850-81 , 010 per LYG ) .
	manualset3
100023	11	400292	5	NULL	NULL	0	NULL	$ 11 , 906-59 , 840 per LYG	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In men aged 40-59 years , the ranking of increasing cost-effectiveness was : smoking cessation ( $ 2 , 608-3 , 738 per LYG ) ; treatment of moderate and severe hypertension ( $ 8 , 564-38 , 678 per LYG ) ; treatment of mild hypertension ( $ 11 , 906-59 , 840 per LYG ) ; dietary treatment ( $ 16 , 143-20 , 158 per LYG ) ; and drug treatment of hypercholesterolemia ( $ 33 , 850-81 , 010 per LYG ) .
	manualset3
100024	12	400292	5	NULL	NULL	0	NULL	dietary treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In men aged 40-59 years , the ranking of increasing cost-effectiveness was : smoking cessation ( $ 2 , 608-3 , 738 per LYG ) ; treatment of moderate and severe hypertension ( $ 8 , 564-38 , 678 per LYG ) ; treatment of mild hypertension ( $ 11 , 906-59 , 840 per LYG ) ; dietary treatment ( $ 16 , 143-20 , 158 per LYG ) ; and drug treatment of hypercholesterolemia ( $ 33 , 850-81 , 010 per LYG ) .
	manualset3
100025	13	400292	5	NULL	NULL	0	NULL	$ 16 , 143-20 , 158 per LYG 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In men aged 40-59 years , the ranking of increasing cost-effectiveness was : smoking cessation ( $ 2 , 608-3 , 738 per LYG ) ; treatment of moderate and severe hypertension ( $ 8 , 564-38 , 678 per LYG ) ; treatment of mild hypertension ( $ 11 , 906-59 , 840 per LYG ) ; dietary treatment ( $ 16 , 143-20 , 158 per LYG ) ; and drug treatment of hypercholesterolemia ( $ 33 , 850-81 , 010 per LYG ) .
	manualset3
100026	14	400292	5	NULL	NULL	0	NULL	drug treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In men aged 40-59 years , the ranking of increasing cost-effectiveness was : smoking cessation ( $ 2 , 608-3 , 738 per LYG ) ; treatment of moderate and severe hypertension ( $ 8 , 564-38 , 678 per LYG ) ; treatment of mild hypertension ( $ 11 , 906-59 , 840 per LYG ) ; dietary treatment ( $ 16 , 143-20 , 158 per LYG ) ; and drug treatment of hypercholesterolemia ( $ 33 , 850-81 , 010 per LYG ) .
	manualset3
100027	15	400292	5	NULL	NULL	NULL	NULL	hypercholesterolemia 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In men aged 40-59 years , the ranking of increasing cost-effectiveness was : smoking cessation ( $ 2 , 608-3 , 738 per LYG ) ; treatment of moderate and severe hypertension ( $ 8 , 564-38 , 678 per LYG ) ; treatment of mild hypertension ( $ 11 , 906-59 , 840 per LYG ) ; dietary treatment ( $ 16 , 143-20 , 158 per LYG ) ; and drug treatment of hypercholesterolemia ( $ 33 , 850-81 , 010 per LYG ) .
	manualset3
100028	16	400292	5	NULL	NULL	0	NULL	 $ 33 , 850-81 , 010 per LYG	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In men aged 40-59 years , the ranking of increasing cost-effectiveness was : smoking cessation ( $ 2 , 608-3 , 738 per LYG ) ; treatment of moderate and severe hypertension ( $ 8 , 564-38 , 678 per LYG ) ; treatment of mild hypertension ( $ 11 , 906-59 , 840 per LYG ) ; dietary treatment ( $ 16 , 143-20 , 158 per LYG ) ; and drug treatment of hypercholesterolemia ( $ 33 , 850-81 , 010 per LYG ) .
	manualset3
100029	1	400293	5	NULL	NULL	0	NULL	mengovirus-infected L cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In mengovirus-infected L cells , 45 S rRNA synthesis , but not processing , is severely inhibited soon after infection , indicating that a decrease in rRNA transcription is not necessarily accompanied by a decrease in processing .
	manualset3
100030	2	400293	5	NULL	NULL	0	NULL	45 S rRNA synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In mengovirus-infected L cells , 45 S rRNA synthesis , but not processing , is severely inhibited soon after infection , indicating that a decrease in rRNA transcription is not necessarily accompanied by a decrease in processing .
	manualset3
100031	3	400293	5	NULL	NULL	0	NULL	processing 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In mengovirus-infected L cells , 45 S rRNA synthesis , but not processing , is severely inhibited soon after infection , indicating that a decrease in rRNA transcription is not necessarily accompanied by a decrease in processing .
	manualset3
100032	4	400293	5	NULL	NULL	NULL	NULL	infection 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In mengovirus-infected L cells , 45 S rRNA synthesis , but not processing , is severely inhibited soon after infection , indicating that a decrease in rRNA transcription is not necessarily accompanied by a decrease in processing .
	manualset3
100033	5	400293	5	NULL	NULL	0	NULL	rRNA transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In mengovirus-infected L cells , 45 S rRNA synthesis , but not processing , is severely inhibited soon after infection , indicating that a decrease in rRNA transcription is not necessarily accompanied by a decrease in processing .
	manualset3
100034	6	400293	5	NULL	NULL	0	NULL	processing 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In mengovirus-infected L cells , 45 S rRNA synthesis , but not processing , is severely inhibited soon after infection , indicating that a decrease in rRNA transcription is not necessarily accompanied by a decrease in processing .
	manualset3
100035	1	400294	5	NULL	NULL	0	NULL	mesenteric artery smooth muscle cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In mesenteric artery smooth muscle cells , depolarizing voltage steps activated outward K + currents whose amplitude was decreased by about 20 % with phenylephrine ( 1-10 microM : n = 14 cells ) .
	manualset3
100036	2	400294	5	NULL	NULL	0	NULL	depolarizing voltage steps	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In mesenteric artery smooth muscle cells , depolarizing voltage steps activated outward K + currents whose amplitude was decreased by about 20 % with phenylephrine ( 1-10 microM : n = 14 cells ) .
	manualset3
100037	3	400294	5	NULL	NULL	0	NULL	outward K + currents	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In mesenteric artery smooth muscle cells , depolarizing voltage steps activated outward K + currents whose amplitude was decreased by about 20 % with phenylephrine ( 1-10 microM : n = 14 cells ) .
	manualset3
100038	4	400294	5	NULL	NULL	0	NULL	amplitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In mesenteric artery smooth muscle cells , depolarizing voltage steps activated outward K + currents whose amplitude was decreased by about 20 % with phenylephrine ( 1-10 microM : n = 14 cells ) .
	manualset3
100039	5	400294	5	NULL	NULL	0	NULL	 20 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In mesenteric artery smooth muscle cells , depolarizing voltage steps activated outward K + currents whose amplitude was decreased by about 20 % with phenylephrine ( 1-10 microM : n = 14 cells ) .
	manualset3
100040	6	400294	5	NULL	NULL	0	NULL	phenylephrine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In mesenteric artery smooth muscle cells , depolarizing voltage steps activated outward K + currents whose amplitude was decreased by about 20 % with phenylephrine ( 1-10 microM : n = 14 cells ) .
	manualset3
100041	7	400294	5	NULL	NULL	NULL	NULL	(1-10 microM : n = 14 cells)	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In mesenteric artery smooth muscle cells , depolarizing voltage steps activated outward K + currents whose amplitude was decreased by about 20 % with phenylephrine ( 1-10 microM : n = 14 cells ) .
	manualset3
100042	1	400295	5	NULL	NULL	NULL	NULL	Deletion 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( i ) Deletion of the cytoplasmic tail , the transmembrane region plus the C-terminal half of the ectodomain of gI , does not affect intracellular transport of gE .
	manualset3
100043	2	400295	5	NULL	NULL	0	NULL	cytoplasmic tail	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	( i ) Deletion of the cytoplasmic tail , the transmembrane region plus the C-terminal half of the ectodomain of gI , does not affect intracellular transport of gE .
	manualset3
100044	3	400295	5	NULL	NULL	0	NULL	transmembrane region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	( i ) Deletion of the cytoplasmic tail , the transmembrane region plus the C-terminal half of the ectodomain of gI , does not affect intracellular transport of gE .
	manualset3
100045	4	400295	5	NULL	NULL	0	NULL	C-terminal half	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	( i ) Deletion of the cytoplasmic tail , the transmembrane region plus the C-terminal half of the ectodomain of gI , does not affect intracellular transport of gE .
	manualset3
100046	5	400295	5	NULL	NULL	0	NULL	ectodomain 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	( i ) Deletion of the cytoplasmic tail , the transmembrane region plus the C-terminal half of the ectodomain of gI , does not affect intracellular transport of gE .
	manualset3
100047	6	400295	5	NULL	NULL	0	NULL	gI	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( i ) Deletion of the cytoplasmic tail , the transmembrane region plus the C-terminal half of the ectodomain of gI , does not affect intracellular transport of gE .
	manualset3
100048	7	400295	5	NULL	NULL	0	NULL	intracellular transport	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( i ) Deletion of the cytoplasmic tail , the transmembrane region plus the C-terminal half of the ectodomain of gI , does not affect intracellular transport of gE .
	manualset3
100049	8	400295	5	NULL	NULL	0	NULL	gE	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( i ) Deletion of the cytoplasmic tail , the transmembrane region plus the C-terminal half of the ectodomain of gI , does not affect intracellular transport of gE .
	manualset3
100050	1	400296	5	NULL	NULL	0	NULL	metabolic acidosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In metabolic acidosis produced by ammonium chloride treatment ( plasma CO2 content = 15.3 + / - 0.8 mequiv .
	manualset3
100051	2	400296	5	NULL	NULL	0	NULL	ammonium chloride treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In metabolic acidosis produced by ammonium chloride treatment ( plasma CO2 content = 15.3 + / - 0.8 mequiv .
	manualset3
100052	3	400296	5	NULL	NULL	0	NULL	plasma CO2 content = 15.3 + / - 0.8 mequiv	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In metabolic acidosis produced by ammonium chloride treatment ( plasma CO2 content = 15.3 + / - 0.8 mequiv .
	manualset3
100053	1	400297	5	NULL	NULL	NULL	NULL	mice exposed to radiation	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In mice exposed to radiation before tumor implantation , the reduced local angiogenic response correlated with significantly reduced growth of tumor cells in vivo .
	manualset3
100054	2	400297	5	NULL	NULL	0	NULL	tumor implantation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In mice exposed to radiation before tumor implantation , the reduced local angiogenic response correlated with significantly reduced growth of tumor cells in vivo .
	manualset3
100055	3	400297	5	NULL	NULL	NULL	NULL	reduced local angiogenic response	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In mice exposed to radiation before tumor implantation , the reduced local angiogenic response correlated with significantly reduced growth of tumor cells in vivo .
	manualset3
100056	4	400297	5	NULL	NULL	0	NULL	significantly reduced growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In mice exposed to radiation before tumor implantation , the reduced local angiogenic response correlated with significantly reduced growth of tumor cells in vivo .
	manualset3
100057	5	400297	5	NULL	NULL	0	NULL	tumor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In mice exposed to radiation before tumor implantation , the reduced local angiogenic response correlated with significantly reduced growth of tumor cells in vivo .
	manualset3
100058	1	400298	5	NULL	NULL	0	NULL	mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In mice preimmunized with spleen cells from I - and/or T-region incompatible donors , leukemia cells were rejected by mice immune only to T-region products , and accepted by mice immune only to I-region products .
	manualset3
100059	2	400298	5	NULL	NULL	0	NULL	spleen cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In mice preimmunized with spleen cells from I - and/or T-region incompatible donors , leukemia cells were rejected by mice immune only to T-region products , and accepted by mice immune only to I-region products .
	manualset3
100060	3	400298	5	NULL	NULL	0	NULL	I - and/or T-region incompatible donors	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In mice preimmunized with spleen cells from I - and/or T-region incompatible donors , leukemia cells were rejected by mice immune only to T-region products , and accepted by mice immune only to I-region products .
	manualset3
100061	4	400298	5	NULL	NULL	0	NULL	leukemia cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In mice preimmunized with spleen cells from I - and/or T-region incompatible donors , leukemia cells were rejected by mice immune only to T-region products , and accepted by mice immune only to I-region products .
	manualset3
100062	5	400298	5	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In mice preimmunized with spleen cells from I - and/or T-region incompatible donors , leukemia cells were rejected by mice immune only to T-region products , and accepted by mice immune only to I-region products .
	manualset3
100063	6	400298	5	NULL	NULL	0	NULL	T-region products	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In mice preimmunized with spleen cells from I - and/or T-region incompatible donors , leukemia cells were rejected by mice immune only to T-region products , and accepted by mice immune only to I-region products .
	manualset3
100064	7	400298	5	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In mice preimmunized with spleen cells from I - and/or T-region incompatible donors , leukemia cells were rejected by mice immune only to T-region products , and accepted by mice immune only to I-region products .
	manualset3
100065	8	400298	5	NULL	NULL	0	NULL	I-region products	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In mice preimmunized with spleen cells from I - and/or T-region incompatible donors , leukemia cells were rejected by mice immune only to T-region products , and accepted by mice immune only to I-region products .
	manualset3
100066	1	400299	5	NULL	NULL	0	NULL	most cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In most cases , equivalent allelic expression was observed ; however , one individual showed CHRNA5 AEI that favored the `` protective '' allele and that was concordant with heterozygosity at polymorphisms 13.5 kb upstream of the CHRNA5 transcription start site .
	manualset3
100067	2	400299	5	NULL	NULL	0	NULL	equivalent allelic expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In most cases , equivalent allelic expression was observed ; however , one individual showed CHRNA5 AEI that favored the `` protective '' allele and that was concordant with heterozygosity at polymorphisms 13.5 kb upstream of the CHRNA5 transcription start site .
	manualset3
100068	3	400299	5	NULL	NULL	0	NULL	one individual	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In most cases , equivalent allelic expression was observed ; however , one individual showed CHRNA5 AEI that favored the `` protective '' allele and that was concordant with heterozygosity at polymorphisms 13.5 kb upstream of the CHRNA5 transcription start site .
	manualset3
100069	4	400299	5	NULL	NULL	NULL	NULL	CHRNA5 AEI	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In most cases , equivalent allelic expression was observed ; however , one individual showed CHRNA5 AEI that favored the `` protective '' allele and that was concordant with heterozygosity at polymorphisms 13.5 kb upstream of the CHRNA5 transcription start site .
	manualset3
100070	5	400299	5	NULL	NULL	0	NULL	`` protective '' allele 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In most cases , equivalent allelic expression was observed ; however , one individual showed CHRNA5 AEI that favored the `` protective '' allele and that was concordant with heterozygosity at polymorphisms 13.5 kb upstream of the CHRNA5 transcription start site .
	manualset3
100071	6	400299	5	NULL	NULL	0	NULL	polymorphisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In most cases , equivalent allelic expression was observed ; however , one individual showed CHRNA5 AEI that favored the `` protective '' allele and that was concordant with heterozygosity at polymorphisms 13.5 kb upstream of the CHRNA5 transcription start site .
	manualset3
100072	7	400299	5	NULL	NULL	0	NULL	13.5 kb	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In most cases , equivalent allelic expression was observed ; however , one individual showed CHRNA5 AEI that favored the `` protective '' allele and that was concordant with heterozygosity at polymorphisms 13.5 kb upstream of the CHRNA5 transcription start site .
	manualset3
100073	8	400299	5	NULL	NULL	0	NULL	CHRNA5 transcription start site	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In most cases , equivalent allelic expression was observed ; however , one individual showed CHRNA5 AEI that favored the `` protective '' allele and that was concordant with heterozygosity at polymorphisms 13.5 kb upstream of the CHRNA5 transcription start site .
	manualset3
109520	9	400299	5	NULL	NULL	0	NULL	heterozygosity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In most cases , equivalent allelic expression was observed ; however , one individual showed CHRNA5 AEI that favored the `` protective '' allele and that was concordant with heterozygosity at polymorphisms 13.5 kb upstream of the CHRNA5 transcription start site .
	manualset3
100074	1	400300	5	NULL	NULL	0	NULL	most cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In most cases , the ectopia affects one or both lower parathyroid glands , although in some instances the two glands on the same side are intrathyroidal .
	manualset3
100075	2	400300	5	NULL	NULL	0	NULL	ectopia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In most cases , the ectopia affects one or both lower parathyroid glands , although in some instances the two glands on the same side are intrathyroidal .
	manualset3
100076	3	400300	5	NULL	NULL	0	NULL	lower parathyroid glands	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In most cases , the ectopia affects one or both lower parathyroid glands , although in some instances the two glands on the same side are intrathyroidal .
	manualset3
100077	4	400300	5	NULL	NULL	0	NULL	two glands 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In most cases , the ectopia affects one or both lower parathyroid glands , although in some instances the two glands on the same side are intrathyroidal .
	manualset3
100078	1	400301	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In most children and adults , chemotherapy is the best strategy followed by allogeneic transplants in those who relapse .
	manualset3
100079	2	400301	5	NULL	NULL	0	NULL	adults 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In most children and adults , chemotherapy is the best strategy followed by allogeneic transplants in those who relapse .
	manualset3
100080	3	400301	5	NULL	NULL	0	NULL	chemotherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In most children and adults , chemotherapy is the best strategy followed by allogeneic transplants in those who relapse .
	manualset3
100081	4	400301	5	NULL	NULL	0	NULL	best strategy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In most children and adults , chemotherapy is the best strategy followed by allogeneic transplants in those who relapse .
	manualset3
100082	5	400301	5	NULL	NULL	0	NULL	allogeneic transplants	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In most children and adults , chemotherapy is the best strategy followed by allogeneic transplants in those who relapse .
	manualset3
100083	1	400302	5	NULL	NULL	0	NULL	mitochondria 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In most mitochondria the matrix contained a paracrystalline material which had a characteristic prismatic shape with a regular internal lattice structure .
	manualset3
100084	2	400302	5	NULL	NULL	0	NULL	matrix 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In most mitochondria the matrix contained a paracrystalline material which had a characteristic prismatic shape with a regular internal lattice structure .
	manualset3
100085	3	400302	5	NULL	NULL	0	NULL	paracrystalline material	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In most mitochondria the matrix contained a paracrystalline material which had a characteristic prismatic shape with a regular internal lattice structure .
	manualset3
100086	4	400302	5	NULL	NULL	0	NULL	prismatic shape	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In most mitochondria the matrix contained a paracrystalline material which had a characteristic prismatic shape with a regular internal lattice structure .
	manualset3
100087	5	400302	5	NULL	NULL	0	NULL	regular internal lattice structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In most mitochondria the matrix contained a paracrystalline material which had a characteristic prismatic shape with a regular internal lattice structure .
	manualset3
100088	1	400303	5	NULL	NULL	0	NULL	nitric oxide synthase inhibitor N omega-nitro-L-arginine methyl ester ( L-NAME , 100 microM )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	( ii ) The nitric oxide synthase inhibitor N omega-nitro-L-arginine methyl ester ( L-NAME , 100 microM ) did not modulate 5-HT-initiated contractions at either level of PO2 .
	manualset3
100089	2	400303	5	NULL	NULL	0	NULL	5-HT-initiated contractions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( ii ) The nitric oxide synthase inhibitor N omega-nitro-L-arginine methyl ester ( L-NAME , 100 microM ) did not modulate 5-HT-initiated contractions at either level of PO2 .
	manualset3
100090	4	400303	5	NULL	NULL	NULL	NULL	PO2	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( ii ) The nitric oxide synthase inhibitor N omega-nitro-L-arginine methyl ester ( L-NAME , 100 microM ) did not modulate 5-HT-initiated contractions at either level of PO2 .
	manualset3
100091	3	400303	5	NULL	NULL	0	NULL	level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( ii ) The nitric oxide synthase inhibitor N omega-nitro-L-arginine methyl ester ( L-NAME , 100 microM ) did not modulate 5-HT-initiated contractions at either level of PO2 .
	manualset3
100092	1	400304	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In most patients , Hashimoto 's thyroiditis can be identified using appropriate clinical and laboratory criteria without resorting to thyroidectomy to differentiate between thyroiditis and a neoplasm .
	manualset3
100093	2	400304	5	NULL	NULL	0	NULL	Hashimoto 's thyroiditis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In most patients , Hashimoto 's thyroiditis can be identified using appropriate clinical and laboratory criteria without resorting to thyroidectomy to differentiate between thyroiditis and a neoplasm .
	manualset3
100094	3	400304	5	NULL	NULL	0	NULL	clinical and laboratory criteria	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In most patients , Hashimoto 's thyroiditis can be identified using appropriate clinical and laboratory criteria without resorting to thyroidectomy to differentiate between thyroiditis and a neoplasm .
	manualset3
100095	4	400304	5	NULL	NULL	0	NULL	thyroidectomy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In most patients , Hashimoto 's thyroiditis can be identified using appropriate clinical and laboratory criteria without resorting to thyroidectomy to differentiate between thyroiditis and a neoplasm .
	manualset3
100096	5	400304	5	NULL	NULL	0	NULL	thyroiditis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In most patients , Hashimoto 's thyroiditis can be identified using appropriate clinical and laboratory criteria without resorting to thyroidectomy to differentiate between thyroiditis and a neoplasm .
	manualset3
100097	6	400304	5	NULL	NULL	0	NULL	neoplasm 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In most patients , Hashimoto 's thyroiditis can be identified using appropriate clinical and laboratory criteria without resorting to thyroidectomy to differentiate between thyroiditis and a neoplasm .
	manualset3
100098	1	400305	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In most patients , MAD treatment had no severe side effect on the signs or symptoms of temporomandibular disorders .
	manualset3
100099	2	400305	5	NULL	NULL	0	NULL	MAD treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In most patients , MAD treatment had no severe side effect on the signs or symptoms of temporomandibular disorders .
	manualset3
100100	3	400305	5	NULL	NULL	0	NULL	severe side effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In most patients , MAD treatment had no severe side effect on the signs or symptoms of temporomandibular disorders .
	manualset3
100101	4	400305	5	NULL	NULL	0	NULL	signs or symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In most patients , MAD treatment had no severe side effect on the signs or symptoms of temporomandibular disorders .
	manualset3
100102	5	400305	5	NULL	NULL	0	NULL	temporomandibular disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In most patients , MAD treatment had no severe side effect on the signs or symptoms of temporomandibular disorders .
	manualset3
100249	1	400306	5	NULL	NULL	0	NULL	multivariate analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analyses , predictors of poor medication adherence were : believing you have diabetes only when your sugar is high ( OR = 7.4 ; 2-27 .2 ) , saying there was no need to take medicine when the glucose was normal ( OR = 3.5 ; 0.9-13 .7 ) , worrying about side-effects of diabetes medicines ( OR = 3.3 ; 1.3-8 .7 ) , lack of self-confidence in controlling diabetes ( OR = 2.8 ; 1.1-7 .1 ) , and feeling medicines are hard to take ( OR = 14.0 ; 4.4-44 .6 ) .
	manualset3
100291	2	400306	5	NULL	NULL	0	NULL	predictors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analyses , predictors of poor medication adherence were : believing you have diabetes only when your sugar is high ( OR = 7.4 ; 2-27 .2 ) , saying there was no need to take medicine when the glucose was normal ( OR = 3.5 ; 0.9-13 .7 ) , worrying about side-effects of diabetes medicines ( OR = 3.3 ; 1.3-8 .7 ) , lack of self-confidence in controlling diabetes ( OR = 2.8 ; 1.1-7 .1 ) , and feeling medicines are hard to take ( OR = 14.0 ; 4.4-44 .6 ) .
	manualset3
100293	3	400306	5	NULL	NULL	0	NULL	poor medication adherence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analyses , predictors of poor medication adherence were : believing you have diabetes only when your sugar is high ( OR = 7.4 ; 2-27 .2 ) , saying there was no need to take medicine when the glucose was normal ( OR = 3.5 ; 0.9-13 .7 ) , worrying about side-effects of diabetes medicines ( OR = 3.3 ; 1.3-8 .7 ) , lack of self-confidence in controlling diabetes ( OR = 2.8 ; 1.1-7 .1 ) , and feeling medicines are hard to take ( OR = 14.0 ; 4.4-44 .6 ) .
	manualset3
100294	4	400306	5	NULL	NULL	0	NULL	diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analyses , predictors of poor medication adherence were : believing you have diabetes only when your sugar is high ( OR = 7.4 ; 2-27 .2 ) , saying there was no need to take medicine when the glucose was normal ( OR = 3.5 ; 0.9-13 .7 ) , worrying about side-effects of diabetes medicines ( OR = 3.3 ; 1.3-8 .7 ) , lack of self-confidence in controlling diabetes ( OR = 2.8 ; 1.1-7 .1 ) , and feeling medicines are hard to take ( OR = 14.0 ; 4.4-44 .6 ) .
	manualset3
100295	5	400306	5	NULL	NULL	0	NULL	sugar	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analyses , predictors of poor medication adherence were : believing you have diabetes only when your sugar is high ( OR = 7.4 ; 2-27 .2 ) , saying there was no need to take medicine when the glucose was normal ( OR = 3.5 ; 0.9-13 .7 ) , worrying about side-effects of diabetes medicines ( OR = 3.3 ; 1.3-8 .7 ) , lack of self-confidence in controlling diabetes ( OR = 2.8 ; 1.1-7 .1 ) , and feeling medicines are hard to take ( OR = 14.0 ; 4.4-44 .6 ) .
	manualset3
100296	6	400306	5	NULL	NULL	0	NULL	OR = 7.4 ; 2-27 .2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analyses , predictors of poor medication adherence were : believing you have diabetes only when your sugar is high ( OR = 7.4 ; 2-27 .2 ) , saying there was no need to take medicine when the glucose was normal ( OR = 3.5 ; 0.9-13 .7 ) , worrying about side-effects of diabetes medicines ( OR = 3.3 ; 1.3-8 .7 ) , lack of self-confidence in controlling diabetes ( OR = 2.8 ; 1.1-7 .1 ) , and feeling medicines are hard to take ( OR = 14.0 ; 4.4-44 .6 ) .
	manualset3
100297	7	400306	5	NULL	NULL	0	NULL	medicine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analyses , predictors of poor medication adherence were : believing you have diabetes only when your sugar is high ( OR = 7.4 ; 2-27 .2 ) , saying there was no need to take medicine when the glucose was normal ( OR = 3.5 ; 0.9-13 .7 ) , worrying about side-effects of diabetes medicines ( OR = 3.3 ; 1.3-8 .7 ) , lack of self-confidence in controlling diabetes ( OR = 2.8 ; 1.1-7 .1 ) , and feeling medicines are hard to take ( OR = 14.0 ; 4.4-44 .6 ) .
	manualset3
100302	8	400306	5	NULL	NULL	0	NULL	glucose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analyses , predictors of poor medication adherence were : believing you have diabetes only when your sugar is high ( OR = 7.4 ; 2-27 .2 ) , saying there was no need to take medicine when the glucose was normal ( OR = 3.5 ; 0.9-13 .7 ) , worrying about side-effects of diabetes medicines ( OR = 3.3 ; 1.3-8 .7 ) , lack of self-confidence in controlling diabetes ( OR = 2.8 ; 1.1-7 .1 ) , and feeling medicines are hard to take ( OR = 14.0 ; 4.4-44 .6 ) .
	manualset3
100303	9	400306	5	NULL	NULL	0	NULL	OR = 3.5 ; 0.9-13 .7	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analyses , predictors of poor medication adherence were : believing you have diabetes only when your sugar is high ( OR = 7.4 ; 2-27 .2 ) , saying there was no need to take medicine when the glucose was normal ( OR = 3.5 ; 0.9-13 .7 ) , worrying about side-effects of diabetes medicines ( OR = 3.3 ; 1.3-8 .7 ) , lack of self-confidence in controlling diabetes ( OR = 2.8 ; 1.1-7 .1 ) , and feeling medicines are hard to take ( OR = 14.0 ; 4.4-44 .6 ) .
	manualset3
100304	10	400306	5	NULL	NULL	0	NULL	side-effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analyses , predictors of poor medication adherence were : believing you have diabetes only when your sugar is high ( OR = 7.4 ; 2-27 .2 ) , saying there was no need to take medicine when the glucose was normal ( OR = 3.5 ; 0.9-13 .7 ) , worrying about side-effects of diabetes medicines ( OR = 3.3 ; 1.3-8 .7 ) , lack of self-confidence in controlling diabetes ( OR = 2.8 ; 1.1-7 .1 ) , and feeling medicines are hard to take ( OR = 14.0 ; 4.4-44 .6 ) .
	manualset3
100305	11	400306	5	NULL	NULL	0	NULL	diabetes medicines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analyses , predictors of poor medication adherence were : believing you have diabetes only when your sugar is high ( OR = 7.4 ; 2-27 .2 ) , saying there was no need to take medicine when the glucose was normal ( OR = 3.5 ; 0.9-13 .7 ) , worrying about side-effects of diabetes medicines ( OR = 3.3 ; 1.3-8 .7 ) , lack of self-confidence in controlling diabetes ( OR = 2.8 ; 1.1-7 .1 ) , and feeling medicines are hard to take ( OR = 14.0 ; 4.4-44 .6 ) .
	manualset3
100307	12	400306	5	NULL	NULL	0	NULL	OR = 3.3 ; 1.3-8 .7	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analyses , predictors of poor medication adherence were : believing you have diabetes only when your sugar is high ( OR = 7.4 ; 2-27 .2 ) , saying there was no need to take medicine when the glucose was normal ( OR = 3.5 ; 0.9-13 .7 ) , worrying about side-effects of diabetes medicines ( OR = 3.3 ; 1.3-8 .7 ) , lack of self-confidence in controlling diabetes ( OR = 2.8 ; 1.1-7 .1 ) , and feeling medicines are hard to take ( OR = 14.0 ; 4.4-44 .6 ) .
	manualset3
100309	13	400306	5	NULL	NULL	0	NULL	lack of self-confidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analyses , predictors of poor medication adherence were : believing you have diabetes only when your sugar is high ( OR = 7.4 ; 2-27 .2 ) , saying there was no need to take medicine when the glucose was normal ( OR = 3.5 ; 0.9-13 .7 ) , worrying about side-effects of diabetes medicines ( OR = 3.3 ; 1.3-8 .7 ) , lack of self-confidence in controlling diabetes ( OR = 2.8 ; 1.1-7 .1 ) , and feeling medicines are hard to take ( OR = 14.0 ; 4.4-44 .6 ) .
	manualset3
100310	14	400306	5	NULL	NULL	0	NULL	diabetes 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analyses , predictors of poor medication adherence were : believing you have diabetes only when your sugar is high ( OR = 7.4 ; 2-27 .2 ) , saying there was no need to take medicine when the glucose was normal ( OR = 3.5 ; 0.9-13 .7 ) , worrying about side-effects of diabetes medicines ( OR = 3.3 ; 1.3-8 .7 ) , lack of self-confidence in controlling diabetes ( OR = 2.8 ; 1.1-7 .1 ) , and feeling medicines are hard to take ( OR = 14.0 ; 4.4-44 .6 ) .
	manualset3
100311	15	400306	5	NULL	NULL	0	NULL	OR = 2.8 ; 1.1-7 .1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analyses , predictors of poor medication adherence were : believing you have diabetes only when your sugar is high ( OR = 7.4 ; 2-27 .2 ) , saying there was no need to take medicine when the glucose was normal ( OR = 3.5 ; 0.9-13 .7 ) , worrying about side-effects of diabetes medicines ( OR = 3.3 ; 1.3-8 .7 ) , lack of self-confidence in controlling diabetes ( OR = 2.8 ; 1.1-7 .1 ) , and feeling medicines are hard to take ( OR = 14.0 ; 4.4-44 .6 ) .
	manualset3
100314	16	400306	5	NULL	NULL	0	NULL	medicines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analyses , predictors of poor medication adherence were : believing you have diabetes only when your sugar is high ( OR = 7.4 ; 2-27 .2 ) , saying there was no need to take medicine when the glucose was normal ( OR = 3.5 ; 0.9-13 .7 ) , worrying about side-effects of diabetes medicines ( OR = 3.3 ; 1.3-8 .7 ) , lack of self-confidence in controlling diabetes ( OR = 2.8 ; 1.1-7 .1 ) , and feeling medicines are hard to take ( OR = 14.0 ; 4.4-44 .6 ) .
	manualset3
100315	17	400306	5	NULL	NULL	0	NULL	OR = 14.0 ; 4.4-44 .6	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analyses , predictors of poor medication adherence were : believing you have diabetes only when your sugar is high ( OR = 7.4 ; 2-27 .2 ) , saying there was no need to take medicine when the glucose was normal ( OR = 3.5 ; 0.9-13 .7 ) , worrying about side-effects of diabetes medicines ( OR = 3.3 ; 1.3-8 .7 ) , lack of self-confidence in controlling diabetes ( OR = 2.8 ; 1.1-7 .1 ) , and feeling medicines are hard to take ( OR = 14.0 ; 4.4-44 .6 ) .
	manualset3
100320	1	400307	5	NULL	NULL	0	NULL	multivariate analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analyses in which group assignment was controlled for , milk volume was positively associated with birth weight but negatively associated with milk energy density .
	manualset3
100321	2	400307	5	NULL	NULL	0	NULL	group assignment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analyses in which group assignment was controlled for , milk volume was positively associated with birth weight but negatively associated with milk energy density .
	manualset3
100323	3	400307	5	NULL	NULL	0	NULL	milk volume 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analyses in which group assignment was controlled for , milk volume was positively associated with birth weight but negatively associated with milk energy density .
	manualset3
100324	4	400307	5	NULL	NULL	0	NULL	birth weight 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analyses in which group assignment was controlled for , milk volume was positively associated with birth weight but negatively associated with milk energy density .
	manualset3
100326	5	400307	5	NULL	NULL	0	NULL	milk energy density 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analyses in which group assignment was controlled for , milk volume was positively associated with birth weight but negatively associated with milk energy density .
	manualset3
100329	1	400308	5	NULL	NULL	0	NULL	multivariate analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analysis ( Cox regression model ) bcl-2 expression remained as an independent prognostic parameter with Dukes ' classification as stratification factor ( P & lt ; 0.001 ) .
	manualset3
100332	2	400308	5	NULL	NULL	0	NULL	Cox regression model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analysis ( Cox regression model ) bcl-2 expression remained as an independent prognostic parameter with Dukes ' classification as stratification factor ( P & lt ; 0.001 ) .
	manualset3
100342	3	400308	5	NULL	NULL	0	NULL	bcl-2 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analysis ( Cox regression model ) bcl-2 expression remained as an independent prognostic parameter with Dukes ' classification as stratification factor ( P & lt ; 0.001 ) .
	manualset3
100343	4	400308	5	NULL	NULL	0	NULL	independent prognostic parameter	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analysis ( Cox regression model ) bcl-2 expression remained as an independent prognostic parameter with Dukes ' classification as stratification factor ( P & lt ; 0.001 ) .
	manualset3
100345	5	400308	5	NULL	NULL	0	NULL	Dukes ' classification 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analysis ( Cox regression model ) bcl-2 expression remained as an independent prognostic parameter with Dukes ' classification as stratification factor ( P & lt ; 0.001 ) .
	manualset3
100347	6	400308	5	NULL	NULL	0	NULL	stratification factor	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analysis ( Cox regression model ) bcl-2 expression remained as an independent prognostic parameter with Dukes ' classification as stratification factor ( P & lt ; 0.001 ) .
	manualset3
100348	7	400308	5	NULL	NULL	0	NULL	P & lt ; 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analysis ( Cox regression model ) bcl-2 expression remained as an independent prognostic parameter with Dukes ' classification as stratification factor ( P & lt ; 0.001 ) .
	manualset3
100357	1	400309	5	NULL	NULL	0	NULL	multivariate analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analysis , prediabetes was associated with insulin resistance and residence in Len .
	manualset3
100359	2	400309	5	NULL	NULL	0	NULL	prediabetes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analysis , prediabetes was associated with insulin resistance and residence in Len .
	manualset3
100364	3	400309	5	NULL	NULL	0	NULL	insulin resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analysis , prediabetes was associated with insulin resistance and residence in Len .
	manualset3
100374	4	400309	5	NULL	NULL	0	NULL	residence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analysis , prediabetes was associated with insulin resistance and residence in Len .
	manualset3
100375	5	400309	5	NULL	NULL	0	NULL	Len	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analysis , prediabetes was associated with insulin resistance and residence in Len .
	manualset3
100376	1	400310	5	NULL	NULL	0	NULL	 multivariate analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analysis , the risk score was a significant risk factor among clinical variables examined together ( hazard ratio ( HR ) , 1.36 ; 95 % confidence interval ( CI ) , 1.13-1 .64 ; P = 0.001 for OS ) .
	manualset3
100377	2	400310	5	NULL	NULL	0	NULL	risk score	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analysis , the risk score was a significant risk factor among clinical variables examined together ( hazard ratio ( HR ) , 1.36 ; 95 % confidence interval ( CI ) , 1.13-1 .64 ; P = 0.001 for OS ) .
	manualset3
100378	3	400310	5	NULL	NULL	0	NULL	significant risk factor	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analysis , the risk score was a significant risk factor among clinical variables examined together ( hazard ratio ( HR ) , 1.36 ; 95 % confidence interval ( CI ) , 1.13-1 .64 ; P = 0.001 for OS ) .
	manualset3
100382	4	400310	5	NULL	NULL	0	NULL	clinical variables	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analysis , the risk score was a significant risk factor among clinical variables examined together ( hazard ratio ( HR ) , 1.36 ; 95 % confidence interval ( CI ) , 1.13-1 .64 ; P = 0.001 for OS ) .
	manualset3
100389	5	400310	5	NULL	NULL	0	NULL	hazard ratio ( HR )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analysis , the risk score was a significant risk factor among clinical variables examined together ( hazard ratio ( HR ) , 1.36 ; 95 % confidence interval ( CI ) , 1.13-1 .64 ; P = 0.001 for OS ) .
	manualset3
100390	6	400310	5	NULL	NULL	0	NULL	1.36	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analysis , the risk score was a significant risk factor among clinical variables examined together ( hazard ratio ( HR ) , 1.36 ; 95 % confidence interval ( CI ) , 1.13-1 .64 ; P = 0.001 for OS ) .
	manualset3
100391	7	400310	5	NULL	NULL	0	NULL	95 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analysis , the risk score was a significant risk factor among clinical variables examined together ( hazard ratio ( HR ) , 1.36 ; 95 % confidence interval ( CI ) , 1.13-1 .64 ; P = 0.001 for OS ) .
	manualset3
100392	8	400310	5	NULL	NULL	0	NULL	confidence interval ( CI )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analysis , the risk score was a significant risk factor among clinical variables examined together ( hazard ratio ( HR ) , 1.36 ; 95 % confidence interval ( CI ) , 1.13-1 .64 ; P = 0.001 for OS ) .
	manualset3
100393	9	400310	5	NULL	NULL	0	NULL	1.13-1 .64	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analysis , the risk score was a significant risk factor among clinical variables examined together ( hazard ratio ( HR ) , 1.36 ; 95 % confidence interval ( CI ) , 1.13-1 .64 ; P = 0.001 for OS ) .
	manualset3
100394	10	400310	5	NULL	NULL	0	NULL	P = 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analysis , the risk score was a significant risk factor among clinical variables examined together ( hazard ratio ( HR ) , 1.36 ; 95 % confidence interval ( CI ) , 1.13-1 .64 ; P = 0.001 for OS ) .
	manualset3
100395	11	400310	5	NULL	NULL	0	NULL	OS	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In multivariate analysis , the risk score was a significant risk factor among clinical variables examined together ( hazard ratio ( HR ) , 1.36 ; 95 % confidence interval ( CI ) , 1.13-1 .64 ; P = 0.001 for OS ) .
	manualset3
100396	1	400311	5	NULL	NULL	0	NULL	muscles 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In muscles and C2C12 myotubes , cholinergic excitation by exposure to nicotine or the organophosphorous pesticide , Paraoxon , induced Tristetraprolin overproduction while reducing pro-inflammatory transcripts such as IL-6 , CXCL1 ( KC ) and CCL2 ( MCP-1 ) .
	manualset3
100397	2	400311	5	NULL	NULL	0	NULL	C2C12 myotubes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In muscles and C2C12 myotubes , cholinergic excitation by exposure to nicotine or the organophosphorous pesticide , Paraoxon , induced Tristetraprolin overproduction while reducing pro-inflammatory transcripts such as IL-6 , CXCL1 ( KC ) and CCL2 ( MCP-1 ) .
	manualset3
100398	3	400311	5	NULL	NULL	0	NULL	cholinergic excitation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In muscles and C2C12 myotubes , cholinergic excitation by exposure to nicotine or the organophosphorous pesticide , Paraoxon , induced Tristetraprolin overproduction while reducing pro-inflammatory transcripts such as IL-6 , CXCL1 ( KC ) and CCL2 ( MCP-1 ) .
	manualset3
100399	4	400311	5	NULL	NULL	0	NULL	exposure 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In muscles and C2C12 myotubes , cholinergic excitation by exposure to nicotine or the organophosphorous pesticide , Paraoxon , induced Tristetraprolin overproduction while reducing pro-inflammatory transcripts such as IL-6 , CXCL1 ( KC ) and CCL2 ( MCP-1 ) .
	manualset3
100400	5	400311	5	NULL	NULL	NULL	NULL	nicotine 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In muscles and C2C12 myotubes , cholinergic excitation by exposure to nicotine or the organophosphorous pesticide , Paraoxon , induced Tristetraprolin overproduction while reducing pro-inflammatory transcripts such as IL-6 , CXCL1 ( KC ) and CCL2 ( MCP-1 ) .
	manualset3
100401	6	400311	5	NULL	NULL	NULL	NULL	organophosphorous pesticide , Paraoxon	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In muscles and C2C12 myotubes , cholinergic excitation by exposure to nicotine or the organophosphorous pesticide , Paraoxon , induced Tristetraprolin overproduction while reducing pro-inflammatory transcripts such as IL-6 , CXCL1 ( KC ) and CCL2 ( MCP-1 ) .
	manualset3
100402	7	400311	5	NULL	NULL	0	NULL	Tristetraprolin overproduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In muscles and C2C12 myotubes , cholinergic excitation by exposure to nicotine or the organophosphorous pesticide , Paraoxon , induced Tristetraprolin overproduction while reducing pro-inflammatory transcripts such as IL-6 , CXCL1 ( KC ) and CCL2 ( MCP-1 ) .
	manualset3
100403	8	400311	5	NULL	NULL	0	NULL	pro-inflammatory transcripts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In muscles and C2C12 myotubes , cholinergic excitation by exposure to nicotine or the organophosphorous pesticide , Paraoxon , induced Tristetraprolin overproduction while reducing pro-inflammatory transcripts such as IL-6 , CXCL1 ( KC ) and CCL2 ( MCP-1 ) .
	manualset3
100405	9	400311	5	NULL	NULL	0	NULL	IL-6	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In muscles and C2C12 myotubes , cholinergic excitation by exposure to nicotine or the organophosphorous pesticide , Paraoxon , induced Tristetraprolin overproduction while reducing pro-inflammatory transcripts such as IL-6 , CXCL1 ( KC ) and CCL2 ( MCP-1 ) .
	manualset3
100406	10	400311	5	NULL	NULL	0	NULL	CXCL1 ( KC )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In muscles and C2C12 myotubes , cholinergic excitation by exposure to nicotine or the organophosphorous pesticide , Paraoxon , induced Tristetraprolin overproduction while reducing pro-inflammatory transcripts such as IL-6 , CXCL1 ( KC ) and CCL2 ( MCP-1 ) .
	manualset3
100408	11	400311	5	NULL	NULL	0	NULL	CCL2 ( MCP-1 )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In muscles and C2C12 myotubes , cholinergic excitation by exposure to nicotine or the organophosphorous pesticide , Paraoxon , induced Tristetraprolin overproduction while reducing pro-inflammatory transcripts such as IL-6 , CXCL1 ( KC ) and CCL2 ( MCP-1 ) .
	manualset3
100412	1	400312	5	NULL	NULL	0	NULL	evasion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In my view , this is an evasion of social responsibility -- social responsibility being one of the hallmarks of an honest profession .
	manualset3
100415	2	400312	5	NULL	NULL	0	NULL	social responsibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In my view , this is an evasion of social responsibility -- social responsibility being one of the hallmarks of an honest profession .
	manualset3
100416	3	400312	5	NULL	NULL	0	NULL	social responsibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In my view , this is an evasion of social responsibility -- social responsibility being one of the hallmarks of an honest profession .
	manualset3
100419	4	400312	5	NULL	NULL	0	NULL	hallmarks	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In my view , this is an evasion of social responsibility -- social responsibility being one of the hallmarks of an honest profession .
	manualset3
100420	5	400312	5	NULL	NULL	0	NULL	honest profession	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In my view , this is an evasion of social responsibility -- social responsibility being one of the hallmarks of an honest profession .
	manualset3
100427	1	400313	5	NULL	NULL	0	NULL	neonatal rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In neonatal rat ventricular myocytes , the alpha-TLR2 antibody inhibited hydrogen peroxide-induced nuclear translocation of NF-kappaB and activator protein-1 ( AP-1 ) .
	manualset3
100428	2	400313	5	NULL	NULL	0	NULL	ventricular myocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In neonatal rat ventricular myocytes , the alpha-TLR2 antibody inhibited hydrogen peroxide-induced nuclear translocation of NF-kappaB and activator protein-1 ( AP-1 ) .
	manualset3
100431	3	400313	5	NULL	NULL	0	NULL	alpha-TLR2 antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In neonatal rat ventricular myocytes , the alpha-TLR2 antibody inhibited hydrogen peroxide-induced nuclear translocation of NF-kappaB and activator protein-1 ( AP-1 ) .
	manualset3
100433	4	400313	5	NULL	NULL	0	NULL	hydrogen peroxide-induced nuclear translocation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In neonatal rat ventricular myocytes , the alpha-TLR2 antibody inhibited hydrogen peroxide-induced nuclear translocation of NF-kappaB and activator protein-1 ( AP-1 ) .
	manualset3
100435	5	400313	5	NULL	NULL	0	NULL	 NF-kappaB	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In neonatal rat ventricular myocytes , the alpha-TLR2 antibody inhibited hydrogen peroxide-induced nuclear translocation of NF-kappaB and activator protein-1 ( AP-1 ) .
	manualset3
100436	6	400313	5	NULL	NULL	0	NULL	activator protein-1 ( AP-1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In neonatal rat ventricular myocytes , the alpha-TLR2 antibody inhibited hydrogen peroxide-induced nuclear translocation of NF-kappaB and activator protein-1 ( AP-1 ) .
	manualset3
100439	1	400314	5	NULL	NULL	0	NULL	Apology	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Apology for the biplane cervico-facial face lift ) .
	manualset3
100440	2	400314	5	NULL	NULL	0	NULL	biplane cervico-facial face lift	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Apology for the biplane cervico-facial face lift ) .
	manualset3
100441	1	400315	5	NULL	NULL	0	NULL	75Se levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( ii ) The sharp decrease of 75Se levels was a prevalent feature of the 75Se kinetics in most of the studied tissues after the injection of the sublethal dose .
	manualset3
100443	2	400315	5	NULL	NULL	0	NULL	prevalent feature	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	( ii ) The sharp decrease of 75Se levels was a prevalent feature of the 75Se kinetics in most of the studied tissues after the injection of the sublethal dose .
	manualset3
100444	3	400315	5	NULL	NULL	NULL	NULL	75Se kinetics	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( ii ) The sharp decrease of 75Se levels was a prevalent feature of the 75Se kinetics in most of the studied tissues after the injection of the sublethal dose .
	manualset3
100447	4	400315	5	NULL	NULL	0	NULL	 studied tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	( ii ) The sharp decrease of 75Se levels was a prevalent feature of the 75Se kinetics in most of the studied tissues after the injection of the sublethal dose .
	manualset3
100448	5	400315	5	NULL	NULL	0	NULL	injection 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( ii ) The sharp decrease of 75Se levels was a prevalent feature of the 75Se kinetics in most of the studied tissues after the injection of the sublethal dose .
	manualset3
100449	6	400315	5	NULL	NULL	0	NULL	sublethal dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( ii ) The sharp decrease of 75Se levels was a prevalent feature of the 75Se kinetics in most of the studied tissues after the injection of the sublethal dose .
	manualset3
100450	1	400316	5	NULL	NULL	0	NULL	neonates	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In neonates and infants with critical aortic coarctation , balloon angioplasty is considered for rescue therapy of heart failure .
	manualset3
100451	2	400316	5	NULL	NULL	0	NULL	infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In neonates and infants with critical aortic coarctation , balloon angioplasty is considered for rescue therapy of heart failure .
	manualset3
100452	3	400316	5	NULL	NULL	0	NULL	critical aortic coarctation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In neonates and infants with critical aortic coarctation , balloon angioplasty is considered for rescue therapy of heart failure .
	manualset3
100454	4	400316	5	NULL	NULL	0	NULL	balloon angioplasty	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In neonates and infants with critical aortic coarctation , balloon angioplasty is considered for rescue therapy of heart failure .
	manualset3
100456	5	400316	5	NULL	NULL	NULL	NULL	rescue therapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In neonates and infants with critical aortic coarctation , balloon angioplasty is considered for rescue therapy of heart failure .
	manualset3
100459	6	400316	5	NULL	NULL	0	NULL	heart failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In neonates and infants with critical aortic coarctation , balloon angioplasty is considered for rescue therapy of heart failure .
	manualset3
100461	1	400317	5	NULL	NULL	0	NULL	neurodegenerative diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In neurodegenerative diseases caused by extended polyglutamine ( polyQ ) sequences in proteins , aggregation-prone polyQ proteins accumulate in intraneuronal inclusions .
	manualset3
100462	2	400317	5	NULL	NULL	0	NULL	extended polyglutamine ( polyQ ) sequences	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In neurodegenerative diseases caused by extended polyglutamine ( polyQ ) sequences in proteins , aggregation-prone polyQ proteins accumulate in intraneuronal inclusions .
	manualset3
100463	3	400317	5	NULL	NULL	0	NULL	proteins 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In neurodegenerative diseases caused by extended polyglutamine ( polyQ ) sequences in proteins , aggregation-prone polyQ proteins accumulate in intraneuronal inclusions .
	manualset3
100464	4	400317	5	NULL	NULL	0	NULL	aggregation-prone polyQ proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In neurodegenerative diseases caused by extended polyglutamine ( polyQ ) sequences in proteins , aggregation-prone polyQ proteins accumulate in intraneuronal inclusions .
	manualset3
100465	5	400317	5	NULL	NULL	0	NULL	intraneuronal inclusions	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In neurodegenerative diseases caused by extended polyglutamine ( polyQ ) sequences in proteins , aggregation-prone polyQ proteins accumulate in intraneuronal inclusions .
	manualset3
100467	1	400318	5	NULL	NULL	0	NULL	neutrophil-like HL-60 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In neutrophil-like HL-60 cells , this asymmetry depends on a positive feedback loop in which accumulation of a membrane lipid , phosphatidylinositol ( PI ) 3 , 4 , 5-trisphosphate ( PI ( 3 , 4 , 5 ) P3 ) , leads to activation of Rac and/or Cdc42 , and vice versa .
	manualset3
100469	2	400318	5	NULL	NULL	0	NULL	asymmetry	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In neutrophil-like HL-60 cells , this asymmetry depends on a positive feedback loop in which accumulation of a membrane lipid , phosphatidylinositol ( PI ) 3 , 4 , 5-trisphosphate ( PI ( 3 , 4 , 5 ) P3 ) , leads to activation of Rac and/or Cdc42 , and vice versa .
	manualset3
100471	3	400318	5	NULL	NULL	0	NULL	positive feedback loop	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In neutrophil-like HL-60 cells , this asymmetry depends on a positive feedback loop in which accumulation of a membrane lipid , phosphatidylinositol ( PI ) 3 , 4 , 5-trisphosphate ( PI ( 3 , 4 , 5 ) P3 ) , leads to activation of Rac and/or Cdc42 , and vice versa .
	manualset3
100472	4	400318	5	NULL	NULL	0	NULL	accumulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In neutrophil-like HL-60 cells , this asymmetry depends on a positive feedback loop in which accumulation of a membrane lipid , phosphatidylinositol ( PI ) 3 , 4 , 5-trisphosphate ( PI ( 3 , 4 , 5 ) P3 ) , leads to activation of Rac and/or Cdc42 , and vice versa .
	manualset3
100475	5	400318	5	NULL	NULL	NULL	NULL	membrane lipid	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In neutrophil-like HL-60 cells , this asymmetry depends on a positive feedback loop in which accumulation of a membrane lipid , phosphatidylinositol ( PI ) 3 , 4 , 5-trisphosphate ( PI ( 3 , 4 , 5 ) P3 ) , leads to activation of Rac and/or Cdc42 , and vice versa .
	manualset3
100477	6	400318	5	NULL	NULL	0	NULL	phosphatidylinositol ( PI ) 3 , 4 , 5-trisphosphate ( PI ( 3 , 4 , 5 ) P3 )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In neutrophil-like HL-60 cells , this asymmetry depends on a positive feedback loop in which accumulation of a membrane lipid , phosphatidylinositol ( PI ) 3 , 4 , 5-trisphosphate ( PI ( 3 , 4 , 5 ) P3 ) , leads to activation of Rac and/or Cdc42 , and vice versa .
	manualset3
100478	7	400318	5	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In neutrophil-like HL-60 cells , this asymmetry depends on a positive feedback loop in which accumulation of a membrane lipid , phosphatidylinositol ( PI ) 3 , 4 , 5-trisphosphate ( PI ( 3 , 4 , 5 ) P3 ) , leads to activation of Rac and/or Cdc42 , and vice versa .
	manualset3
100479	8	400318	5	NULL	NULL	0	NULL	Rac	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In neutrophil-like HL-60 cells , this asymmetry depends on a positive feedback loop in which accumulation of a membrane lipid , phosphatidylinositol ( PI ) 3 , 4 , 5-trisphosphate ( PI ( 3 , 4 , 5 ) P3 ) , leads to activation of Rac and/or Cdc42 , and vice versa .
	manualset3
100480	9	400318	5	NULL	NULL	0	NULL	Cdc42	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In neutrophil-like HL-60 cells , this asymmetry depends on a positive feedback loop in which accumulation of a membrane lipid , phosphatidylinositol ( PI ) 3 , 4 , 5-trisphosphate ( PI ( 3 , 4 , 5 ) P3 ) , leads to activation of Rac and/or Cdc42 , and vice versa .
	manualset3
100481	1	400319	5	NULL	NULL	0	NULL	nine patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In nine patients ( including three patients with a previous history of asthma ) with pre-operative BHR ( defined as PD20 His & lt ; 2 mg ) , mean PD20 His did not change significantly at 6 weeks , nor at 6 months after TS ( 0.62 + / - 0.33 , 0.71 + / - 0.42 and 0.93 + / - 0.65 mg , respectively ) although there was a non-significant trend towards an increase in PD20 His at 6 months .
	manualset3
100483	2	400319	5	NULL	NULL	0	NULL	 three patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In nine patients ( including three patients with a previous history of asthma ) with pre-operative BHR ( defined as PD20 His & lt ; 2 mg ) , mean PD20 His did not change significantly at 6 weeks , nor at 6 months after TS ( 0.62 + / - 0.33 , 0.71 + / - 0.42 and 0.93 + / - 0.65 mg , respectively ) although there was a non-significant trend towards an increase in PD20 His at 6 months .
	manualset3
100488	3	400319	5	NULL	NULL	0	NULL	previous history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In nine patients ( including three patients with a previous history of asthma ) with pre-operative BHR ( defined as PD20 His & lt ; 2 mg ) , mean PD20 His did not change significantly at 6 weeks , nor at 6 months after TS ( 0.62 + / - 0.33 , 0.71 + / - 0.42 and 0.93 + / - 0.65 mg , respectively ) although there was a non-significant trend towards an increase in PD20 His at 6 months .
	manualset3
100489	4	400319	5	NULL	NULL	0	NULL	asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In nine patients ( including three patients with a previous history of asthma ) with pre-operative BHR ( defined as PD20 His & lt ; 2 mg ) , mean PD20 His did not change significantly at 6 weeks , nor at 6 months after TS ( 0.62 + / - 0.33 , 0.71 + / - 0.42 and 0.93 + / - 0.65 mg , respectively ) although there was a non-significant trend towards an increase in PD20 His at 6 months .
	manualset3
100490	5	400319	5	NULL	NULL	NULL	NULL	pre-operative BHR	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In nine patients ( including three patients with a previous history of asthma ) with pre-operative BHR ( defined as PD20 His & lt ; 2 mg ) , mean PD20 His did not change significantly at 6 weeks , nor at 6 months after TS ( 0.62 + / - 0.33 , 0.71 + / - 0.42 and 0.93 + / - 0.65 mg , respectively ) although there was a non-significant trend towards an increase in PD20 His at 6 months .
	manualset3
100510	6	400319	5	NULL	NULL	NULL	NULL	PD20 His	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In nine patients ( including three patients with a previous history of asthma ) with pre-operative BHR ( defined as PD20 His & lt ; 2 mg ) , mean PD20 His did not change significantly at 6 weeks , nor at 6 months after TS ( 0.62 + / - 0.33 , 0.71 + / - 0.42 and 0.93 + / - 0.65 mg , respectively ) although there was a non-significant trend towards an increase in PD20 His at 6 months .
	manualset3
100512	7	400319	5	NULL	NULL	0	NULL	mean PD20 His	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In nine patients ( including three patients with a previous history of asthma ) with pre-operative BHR ( defined as PD20 His & lt ; 2 mg ) , mean PD20 His did not change significantly at 6 weeks , nor at 6 months after TS ( 0.62 + / - 0.33 , 0.71 + / - 0.42 and 0.93 + / - 0.65 mg , respectively ) although there was a non-significant trend towards an increase in PD20 His at 6 months .
	manualset3
100513	8	400319	5	NULL	NULL	0	NULL	6 weeks	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In nine patients ( including three patients with a previous history of asthma ) with pre-operative BHR ( defined as PD20 His & lt ; 2 mg ) , mean PD20 His did not change significantly at 6 weeks , nor at 6 months after TS ( 0.62 + / - 0.33 , 0.71 + / - 0.42 and 0.93 + / - 0.65 mg , respectively ) although there was a non-significant trend towards an increase in PD20 His at 6 months .
	manualset3
100514	9	400319	5	NULL	NULL	0	NULL	6 months	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In nine patients ( including three patients with a previous history of asthma ) with pre-operative BHR ( defined as PD20 His & lt ; 2 mg ) , mean PD20 His did not change significantly at 6 weeks , nor at 6 months after TS ( 0.62 + / - 0.33 , 0.71 + / - 0.42 and 0.93 + / - 0.65 mg , respectively ) although there was a non-significant trend towards an increase in PD20 His at 6 months .
	manualset3
100515	10	400319	5	NULL	NULL	NULL	NULL	TS	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In nine patients ( including three patients with a previous history of asthma ) with pre-operative BHR ( defined as PD20 His & lt ; 2 mg ) , mean PD20 His did not change significantly at 6 weeks , nor at 6 months after TS ( 0.62 + / - 0.33 , 0.71 + / - 0.42 and 0.93 + / - 0.65 mg , respectively ) although there was a non-significant trend towards an increase in PD20 His at 6 months .
	manualset3
100516	11	400319	5	NULL	NULL	0	NULL	0.62 + / - 0.33	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In nine patients ( including three patients with a previous history of asthma ) with pre-operative BHR ( defined as PD20 His & lt ; 2 mg ) , mean PD20 His did not change significantly at 6 weeks , nor at 6 months after TS ( 0.62 + / - 0.33 , 0.71 + / - 0.42 and 0.93 + / - 0.65 mg , respectively ) although there was a non-significant trend towards an increase in PD20 His at 6 months .
	manualset3
100517	12	400319	5	NULL	NULL	0	NULL	0.71 + / - 0.42	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In nine patients ( including three patients with a previous history of asthma ) with pre-operative BHR ( defined as PD20 His & lt ; 2 mg ) , mean PD20 His did not change significantly at 6 weeks , nor at 6 months after TS ( 0.62 + / - 0.33 , 0.71 + / - 0.42 and 0.93 + / - 0.65 mg , respectively ) although there was a non-significant trend towards an increase in PD20 His at 6 months .
	manualset3
100518	13	400319	5	NULL	NULL	0	NULL	0.93 + / - 0.65 mg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In nine patients ( including three patients with a previous history of asthma ) with pre-operative BHR ( defined as PD20 His & lt ; 2 mg ) , mean PD20 His did not change significantly at 6 weeks , nor at 6 months after TS ( 0.62 + / - 0.33 , 0.71 + / - 0.42 and 0.93 + / - 0.65 mg , respectively ) although there was a non-significant trend towards an increase in PD20 His at 6 months .
	manualset3
100519	14	400319	5	NULL	NULL	0	NULL	non-significant trend	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In nine patients ( including three patients with a previous history of asthma ) with pre-operative BHR ( defined as PD20 His & lt ; 2 mg ) , mean PD20 His did not change significantly at 6 weeks , nor at 6 months after TS ( 0.62 + / - 0.33 , 0.71 + / - 0.42 and 0.93 + / - 0.65 mg , respectively ) although there was a non-significant trend towards an increase in PD20 His at 6 months .
	manualset3
100520	15	400319	5	NULL	NULL	0	NULL	PD20 His	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In nine patients ( including three patients with a previous history of asthma ) with pre-operative BHR ( defined as PD20 His & lt ; 2 mg ) , mean PD20 His did not change significantly at 6 weeks , nor at 6 months after TS ( 0.62 + / - 0.33 , 0.71 + / - 0.42 and 0.93 + / - 0.65 mg , respectively ) although there was a non-significant trend towards an increase in PD20 His at 6 months .
	manualset3
100521	16	400319	5	NULL	NULL	0	NULL	6 months	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In nine patients ( including three patients with a previous history of asthma ) with pre-operative BHR ( defined as PD20 His & lt ; 2 mg ) , mean PD20 His did not change significantly at 6 weeks , nor at 6 months after TS ( 0.62 + / - 0.33 , 0.71 + / - 0.42 and 0.93 + / - 0.65 mg , respectively ) although there was a non-significant trend towards an increase in PD20 His at 6 months .
	manualset3
100522	17	400319	5	NULL	NULL	0	NULL	lt ; 2 mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In nine patients ( including three patients with a previous history of asthma ) with pre-operative BHR ( defined as PD20 His & lt ; 2 mg ) , mean PD20 His did not change significantly at 6 weeks , nor at 6 months after TS ( 0.62 + / - 0.33 , 0.71 + / - 0.42 and 0.93 + / - 0.65 mg , respectively ) although there was a non-significant trend towards an increase in PD20 His at 6 months .
	manualset3
100523	1	400320	5	NULL	NULL	0	NULL	non-injured adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In non-injured adults , 30min of repetitive common peroneal nerve stimulation ( rCPnS ) increases CST excitability by 40-50 % and the effect persists for at least 30min .
	manualset3
100524	2	400320	5	NULL	NULL	0	NULL	30min 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In non-injured adults , 30min of repetitive common peroneal nerve stimulation ( rCPnS ) increases CST excitability by 40-50 % and the effect persists for at least 30min .
	manualset3
100525	3	400320	5	NULL	NULL	0	NULL	repetitive common peroneal nerve stimulation ( rCPnS )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In non-injured adults , 30min of repetitive common peroneal nerve stimulation ( rCPnS ) increases CST excitability by 40-50 % and the effect persists for at least 30min .
	manualset3
100526	4	400320	5	NULL	NULL	0	NULL	CST excitability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In non-injured adults , 30min of repetitive common peroneal nerve stimulation ( rCPnS ) increases CST excitability by 40-50 % and the effect persists for at least 30min .
	manualset3
100527	5	400320	5	NULL	NULL	0	NULL	40-50 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In non-injured adults , 30min of repetitive common peroneal nerve stimulation ( rCPnS ) increases CST excitability by 40-50 % and the effect persists for at least 30min .
	manualset3
100528	6	400320	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In non-injured adults , 30min of repetitive common peroneal nerve stimulation ( rCPnS ) increases CST excitability by 40-50 % and the effect persists for at least 30min .
	manualset3
100529	7	400320	5	NULL	NULL	0	NULL	30min	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In non-injured adults , 30min of repetitive common peroneal nerve stimulation ( rCPnS ) increases CST excitability by 40-50 % and the effect persists for at least 30min .
	manualset3
100560	1	400321	5	NULL	NULL	0	NULL	nondenaturing gels	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In nondenaturing gels , anti-c-neu antibody identified high molecular weight proteins ( about 300-400 kDa ) that were reduced by EDTA to a molecular weight of 180-200 kDa .
	manualset3
100561	2	400321	5	NULL	NULL	0	NULL	anti-c-neu antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In nondenaturing gels , anti-c-neu antibody identified high molecular weight proteins ( about 300-400 kDa ) that were reduced by EDTA to a molecular weight of 180-200 kDa .
	manualset3
100562	3	400321	5	NULL	NULL	0	NULL	high molecular weight proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In nondenaturing gels , anti-c-neu antibody identified high molecular weight proteins ( about 300-400 kDa ) that were reduced by EDTA to a molecular weight of 180-200 kDa .
	manualset3
100564	4	400321	5	NULL	NULL	0	NULL	about 300-400 kDa	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In nondenaturing gels , anti-c-neu antibody identified high molecular weight proteins ( about 300-400 kDa ) that were reduced by EDTA to a molecular weight of 180-200 kDa .
	manualset3
100569	5	400321	5	NULL	NULL	0	NULL	EDTA	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In nondenaturing gels , anti-c-neu antibody identified high molecular weight proteins ( about 300-400 kDa ) that were reduced by EDTA to a molecular weight of 180-200 kDa .
	manualset3
100570	6	400321	5	NULL	NULL	0	NULL	molecular weight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In nondenaturing gels , anti-c-neu antibody identified high molecular weight proteins ( about 300-400 kDa ) that were reduced by EDTA to a molecular weight of 180-200 kDa .
	manualset3
100571	7	400321	5	NULL	NULL	0	NULL	180-200 kDa	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In nondenaturing gels , anti-c-neu antibody identified high molecular weight proteins ( about 300-400 kDa ) that were reduced by EDTA to a molecular weight of 180-200 kDa .
	manualset3
100573	1	400322	5	NULL	NULL	0	NULL	normal air	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal air , VE was also significantly elevated in B6 , but not C3 , mice after O3 .
	manualset3
100578	2	400322	5	NULL	NULL	0	NULL	VE	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal air , VE was also significantly elevated in B6 , but not C3 , mice after O3 .
	manualset3
100579	3	400322	5	NULL	NULL	0	NULL	B6 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal air , VE was also significantly elevated in B6 , but not C3 , mice after O3 .
	manualset3
100581	4	400322	5	NULL	NULL	0	NULL	C3 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal air , VE was also significantly elevated in B6 , but not C3 , mice after O3 .
	manualset3
100586	5	400322	5	NULL	NULL	0	NULL	O3	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal air , VE was also significantly elevated in B6 , but not C3 , mice after O3 .
	manualset3
100608	1	400323	5	NULL	NULL	0	NULL	normal human adult eyes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal human adult eyes , immunostaining for tenascin-X was seen in the anterior one-third stroma of cornea , in the stroma of limbus and conjunctiva , and in blood vessels .
	manualset3
100610	2	400323	5	NULL	NULL	0	NULL	immunostaining 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal human adult eyes , immunostaining for tenascin-X was seen in the anterior one-third stroma of cornea , in the stroma of limbus and conjunctiva , and in blood vessels .
	manualset3
100612	3	400323	5	NULL	NULL	0	NULL	tenascin-X 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal human adult eyes , immunostaining for tenascin-X was seen in the anterior one-third stroma of cornea , in the stroma of limbus and conjunctiva , and in blood vessels .
	manualset3
100614	4	400323	5	NULL	NULL	0	NULL	anterior one-third stroma of cornea	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal human adult eyes , immunostaining for tenascin-X was seen in the anterior one-third stroma of cornea , in the stroma of limbus and conjunctiva , and in blood vessels .
	manualset3
100615	5	400323	5	NULL	NULL	NULL	NULL	stroma of limbus 	AnatomicalPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In normal human adult eyes , immunostaining for tenascin-X was seen in the anterior one-third stroma of cornea , in the stroma of limbus and conjunctiva , and in blood vessels .
	manualset3
100618	6	400323	5	NULL	NULL	0	NULL	stroma of conjunctiva	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal human adult eyes , immunostaining for tenascin-X was seen in the anterior one-third stroma of cornea , in the stroma of limbus and conjunctiva , and in blood vessels .
	manualset3
100619	7	400323	5	NULL	NULL	0	NULL	blood vessels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal human adult eyes , immunostaining for tenascin-X was seen in the anterior one-third stroma of cornea , in the stroma of limbus and conjunctiva , and in blood vessels .
	manualset3
100620	1	400324	5	NULL	NULL	0	NULL	normal weight mothers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal weight ( n = 153 ) mothers , higher intake of soft drinks was the strongest predictor of higher offspring WFA at birth ( beta = 0.16 ; P = 0.04 ) but not at 6 months .
	manualset3
100621	2	400324	5	NULL	NULL	0	NULL	( n = 153 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal weight ( n = 153 ) mothers , higher intake of soft drinks was the strongest predictor of higher offspring WFA at birth ( beta = 0.16 ; P = 0.04 ) but not at 6 months .
	manualset3
100622	3	400324	5	NULL	NULL	0	NULL	higher intake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal weight ( n = 153 ) mothers , higher intake of soft drinks was the strongest predictor of higher offspring WFA at birth ( beta = 0.16 ; P = 0.04 ) but not at 6 months .
	manualset3
100623	4	400324	5	NULL	NULL	0	NULL	soft drinks	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal weight ( n = 153 ) mothers , higher intake of soft drinks was the strongest predictor of higher offspring WFA at birth ( beta = 0.16 ; P = 0.04 ) but not at 6 months .
	manualset3
100624	5	400324	5	NULL	NULL	0	NULL	strongest predictor 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal weight ( n = 153 ) mothers , higher intake of soft drinks was the strongest predictor of higher offspring WFA at birth ( beta = 0.16 ; P = 0.04 ) but not at 6 months .
	manualset3
100625	6	400324	5	NULL	NULL	0	NULL	higher offspring WFA	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal weight ( n = 153 ) mothers , higher intake of soft drinks was the strongest predictor of higher offspring WFA at birth ( beta = 0.16 ; P = 0.04 ) but not at 6 months .
	manualset3
100626	7	400324	5	NULL	NULL	0	NULL	birth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal weight ( n = 153 ) mothers , higher intake of soft drinks was the strongest predictor of higher offspring WFA at birth ( beta = 0.16 ; P = 0.04 ) but not at 6 months .
	manualset3
100628	8	400324	5	NULL	NULL	0	NULL	( beta = 0.16 ; P = 0.04 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal weight ( n = 153 ) mothers , higher intake of soft drinks was the strongest predictor of higher offspring WFA at birth ( beta = 0.16 ; P = 0.04 ) but not at 6 months .
	manualset3
100630	9	400324	5	NULL	NULL	0	NULL	6 months	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal weight ( n = 153 ) mothers , higher intake of soft drinks was the strongest predictor of higher offspring WFA at birth ( beta = 0.16 ; P = 0.04 ) but not at 6 months .
	manualset3
100640	1	400325	5	NULL	NULL	0	NULL	nuclear medicine	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In nuclear medicine , an important advance was the application of spect in the diagnosis and localisation of disturbances of regional myocardial perfusion in coronary heart disease .
	manualset3
100641	2	400325	5	NULL	NULL	0	NULL	application 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In nuclear medicine , an important advance was the application of spect in the diagnosis and localisation of disturbances of regional myocardial perfusion in coronary heart disease .
	manualset3
100642	3	400325	5	NULL	NULL	0	NULL	spect 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In nuclear medicine , an important advance was the application of spect in the diagnosis and localisation of disturbances of regional myocardial perfusion in coronary heart disease .
	manualset3
100643	4	400325	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In nuclear medicine , an important advance was the application of spect in the diagnosis and localisation of disturbances of regional myocardial perfusion in coronary heart disease .
	manualset3
100644	5	400325	5	NULL	NULL	0	NULL	localisation of disturbances of regional myocardial perfusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In nuclear medicine , an important advance was the application of spect in the diagnosis and localisation of disturbances of regional myocardial perfusion in coronary heart disease .
	manualset3
100645	6	400325	5	NULL	NULL	0	NULL	coronary heart disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In nuclear medicine , an important advance was the application of spect in the diagnosis and localisation of disturbances of regional myocardial perfusion in coronary heart disease .
	manualset3
100646	1	400326	5	NULL	NULL	0	NULL	( n = 5 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( n = 5 ) , or vehicle ( n = 5 ) for 10 consecutive days .
	manualset3
100647	2	400326	5	NULL	NULL	NULL	NULL	vehicle 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( n = 5 ) , or vehicle ( n = 5 ) for 10 consecutive days .
	manualset3
100648	3	400326	5	NULL	NULL	0	NULL	( n = 5 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( n = 5 ) , or vehicle ( n = 5 ) for 10 consecutive days .
	manualset3
100649	4	400326	5	NULL	NULL	0	NULL	10 consecutive days	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	( n = 5 ) , or vehicle ( n = 5 ) for 10 consecutive days .
	manualset3
100650	1	400327	5	NULL	NULL	0	NULL	older adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In older adults , higher indices of attentional distraction as well as lower conflict monitoring signals were observed .
	manualset3
100651	2	400327	5	NULL	NULL	0	NULL	higher indices	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In older adults , higher indices of attentional distraction as well as lower conflict monitoring signals were observed .
	manualset3
100652	3	400327	5	NULL	NULL	0	NULL	attentional distraction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In older adults , higher indices of attentional distraction as well as lower conflict monitoring signals were observed .
	manualset3
100653	4	400327	5	NULL	NULL	0	NULL	lower conflict monitoring signals	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In older adults , higher indices of attentional distraction as well as lower conflict monitoring signals were observed .
	manualset3
100654	1	400328	5	NULL	NULL	0	NULL	50 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In one , 50 patients with a confirmed diagnosis of typhoid fever .
	manualset3
100656	2	400328	5	NULL	NULL	0	NULL	confirmed diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In one , 50 patients with a confirmed diagnosis of typhoid fever .
	manualset3
100657	3	400328	5	NULL	NULL	0	NULL	typhoid fever	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In one , 50 patients with a confirmed diagnosis of typhoid fever .
	manualset3
100658	1	400329	5	NULL	NULL	0	NULL	one method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In one method , daily increasing dose method ( DIDM ) , a single antigen challenge was performed every day successively .
	manualset3
100659	2	400329	5	NULL	NULL	0	NULL	daily increasing dose method ( DIDM )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In one method , daily increasing dose method ( DIDM ) , a single antigen challenge was performed every day successively .
	manualset3
100660	3	400329	5	NULL	NULL	0	NULL	single antigen challenge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In one method , daily increasing dose method ( DIDM ) , a single antigen challenge was performed every day successively .
	manualset3
100661	4	400329	5	NULL	NULL	0	NULL	every day	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In one method , daily increasing dose method ( DIDM ) , a single antigen challenge was performed every day successively .
	manualset3
100662	1	400330	5	NULL	NULL	0	NULL	reports 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In one of these reports , inorganic salts and chloramine-T were delivered subgingivally throughout root-planing procedures , in addition to home application of inorganic salts .
	manualset3
100663	2	400330	5	NULL	NULL	0	NULL	inorganic salts	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In one of these reports , inorganic salts and chloramine-T were delivered subgingivally throughout root-planing procedures , in addition to home application of inorganic salts .
	manualset3
100664	3	400330	5	NULL	NULL	0	NULL	chloramine-T	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In one of these reports , inorganic salts and chloramine-T were delivered subgingivally throughout root-planing procedures , in addition to home application of inorganic salts .
	manualset3
100665	4	400330	5	NULL	NULL	NULL	NULL	root-planing procedures	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In one of these reports , inorganic salts and chloramine-T were delivered subgingivally throughout root-planing procedures , in addition to home application of inorganic salts .
	manualset3
100666	5	400330	5	NULL	NULL	0	NULL	home application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In one of these reports , inorganic salts and chloramine-T were delivered subgingivally throughout root-planing procedures , in addition to home application of inorganic salts .
	manualset3
100667	6	400330	5	NULL	NULL	0	NULL	inorganic salts	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In one of these reports , inorganic salts and chloramine-T were delivered subgingivally throughout root-planing procedures , in addition to home application of inorganic salts .
	manualset3
100874	1	400331	5	NULL	NULL	0	NULL	re-entry	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order for re-entry to occur , an area of slowing conduction combined with unidirectional block must be present .
	manualset3
100875	2	400331	5	NULL	NULL	0	NULL	area of slowing conduction	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In order for re-entry to occur , an area of slowing conduction combined with unidirectional block must be present .
	manualset3
100876	3	400331	5	NULL	NULL	NULL	NULL	unidirectional block	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In order for re-entry to occur , an area of slowing conduction combined with unidirectional block must be present .
	manualset3
100877	1	400332	5	NULL	NULL	0	NULL	Verongida	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( order Verongida , family Aplysinellidae ) , exhibited potent IC ( 50 ) values of 0.4 and 0.1 microg/mL , respectively .
	manualset3
100878	2	400332	5	NULL	NULL	0	NULL	family Aplysinellidae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( order Verongida , family Aplysinellidae ) , exhibited potent IC ( 50 ) values of 0.4 and 0.1 microg/mL , respectively .
	manualset3
100879	3	400332	5	NULL	NULL	NULL	NULL	potent IC (50) values	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( order Verongida , family Aplysinellidae ) , exhibited potent IC ( 50 ) values of 0.4 and 0.1 microg/mL , respectively .
	manualset3
100880	4	400332	5	NULL	NULL	0	NULL	 0.4 microg/mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( order Verongida , family Aplysinellidae ) , exhibited potent IC ( 50 ) values of 0.4 and 0.1 microg/mL , respectively .
	manualset3
100881	5	400332	5	NULL	NULL	0	NULL	0.1 microg/mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( order Verongida , family Aplysinellidae ) , exhibited potent IC ( 50 ) values of 0.4 and 0.1 microg/mL , respectively .
	manualset3
100888	1	400333	5	NULL	NULL	0	NULL	gene expression data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In order for the gene expression data to be linked with tooth type determination , it is first necessary to determine precisely the incisor - , canine - , premolar - , and molar-forming regions in the jaw primordia .
	manualset3
100889	2	400333	5	NULL	NULL	0	NULL	tooth type determination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In order for the gene expression data to be linked with tooth type determination , it is first necessary to determine precisely the incisor - , canine - , premolar - , and molar-forming regions in the jaw primordia .
	manualset3
100890	3	400333	5	NULL	NULL	NULL	NULL	incisor - forming regions	AnatomicalPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In order for the gene expression data to be linked with tooth type determination , it is first necessary to determine precisely the incisor - , canine - , premolar - , and molar-forming regions in the jaw primordia .
	manualset3
100891	4	400333	5	NULL	NULL	NULL	NULL	canine - forming regions	AnatomicalPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In order for the gene expression data to be linked with tooth type determination , it is first necessary to determine precisely the incisor - , canine - , premolar - , and molar-forming regions in the jaw primordia .
	manualset3
100892	5	400333	5	NULL	NULL	NULL	NULL	premolar - forming regions	AnatomicalPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In order for the gene expression data to be linked with tooth type determination , it is first necessary to determine precisely the incisor - , canine - , premolar - , and molar-forming regions in the jaw primordia .
	manualset3
100893	6	400333	5	NULL	NULL	NULL	NULL	molar-forming regions	AnatomicalPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In order for the gene expression data to be linked with tooth type determination , it is first necessary to determine precisely the incisor - , canine - , premolar - , and molar-forming regions in the jaw primordia .
	manualset3
100894	7	400333	5	NULL	NULL	NULL	NULL	jaw primordia	AnatomicalPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In order for the gene expression data to be linked with tooth type determination , it is first necessary to determine precisely the incisor - , canine - , premolar - , and molar-forming regions in the jaw primordia .
	manualset3
100895	1	400334	5	NULL	NULL	0	NULL	patient satisfaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to achieve a greater impact on patient satisfaction , a combination of information sources in the out-patient department should be targeted at young adults with chronic diseases .
	manualset3
100896	2	400334	5	NULL	NULL	0	NULL	information sources	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to achieve a greater impact on patient satisfaction , a combination of information sources in the out-patient department should be targeted at young adults with chronic diseases .
	manualset3
100897	3	400334	5	NULL	NULL	0	NULL	out-patient department 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to achieve a greater impact on patient satisfaction , a combination of information sources in the out-patient department should be targeted at young adults with chronic diseases .
	manualset3
100898	4	400334	5	NULL	NULL	0	NULL	 young adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to achieve a greater impact on patient satisfaction , a combination of information sources in the out-patient department should be targeted at young adults with chronic diseases .
	manualset3
100899	5	400334	5	NULL	NULL	0	NULL	chronic diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to achieve a greater impact on patient satisfaction , a combination of information sources in the out-patient department should be targeted at young adults with chronic diseases .
	manualset3
100900	1	400335	5	NULL	NULL	NULL	NULL	hostile host environment	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In order to adapt to and to cope with an often hostile host environment , many viruses have evolved to encode products that are homologous to cellular proteins .
	manualset3
100901	2	400335	5	NULL	NULL	0	NULL	viruses 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to adapt to and to cope with an often hostile host environment , many viruses have evolved to encode products that are homologous to cellular proteins .
	manualset3
100902	3	400335	5	NULL	NULL	NULL	NULL	products 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In order to adapt to and to cope with an often hostile host environment , many viruses have evolved to encode products that are homologous to cellular proteins .
	manualset3
100903	4	400335	5	NULL	NULL	NULL	NULL	cellular proteins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In order to adapt to and to cope with an often hostile host environment , many viruses have evolved to encode products that are homologous to cellular proteins .
	manualset3
100904	1	400336	5	NULL	NULL	0	NULL	specific cell adhesion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to allow specific cell adhesion the films were modified with linear RGD peptides ( gRGDsc ) in different concentrations .
	manualset3
100905	2	400336	5	NULL	NULL	0	NULL	films	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to allow specific cell adhesion the films were modified with linear RGD peptides ( gRGDsc ) in different concentrations .
	manualset3
100906	3	400336	5	NULL	NULL	0	NULL	linear RGD peptides ( gRGDsc )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to allow specific cell adhesion the films were modified with linear RGD peptides ( gRGDsc ) in different concentrations .
	manualset3
100907	4	400336	5	NULL	NULL	0	NULL	different concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to allow specific cell adhesion the films were modified with linear RGD peptides ( gRGDsc ) in different concentrations .
	manualset3
100908	1	400337	5	NULL	NULL	0	NULL	contribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to assess the contribution of individual components to the disease , highly pure allergen preparations are required .
	manualset3
100909	2	400337	5	NULL	NULL	0	NULL	 individual components	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to assess the contribution of individual components to the disease , highly pure allergen preparations are required .
	manualset3
100910	3	400337	5	NULL	NULL	0	NULL	disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to assess the contribution of individual components to the disease , highly pure allergen preparations are required .
	manualset3
100911	4	400337	5	NULL	NULL	0	NULL	highly pure allergen preparations	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to assess the contribution of individual components to the disease , highly pure allergen preparations are required .
	manualset3
100912	1	400338	5	NULL	NULL	0	NULL	optimization 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to automate the optimization of complex biochemical and molecular biology reactions , we developed a sequential injection analysis ( SIA ) device and combined this with a design of experiment ( DOE ) algorithm .
	manualset3
100913	2	400338	5	NULL	NULL	0	NULL	complex biochemical and molecular biology reactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to automate the optimization of complex biochemical and molecular biology reactions , we developed a sequential injection analysis ( SIA ) device and combined this with a design of experiment ( DOE ) algorithm .
	manualset3
100914	3	400338	5	NULL	NULL	0	NULL	sequential injection analysis ( SIA ) device	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to automate the optimization of complex biochemical and molecular biology reactions , we developed a sequential injection analysis ( SIA ) device and combined this with a design of experiment ( DOE ) algorithm .
	manualset3
100915	4	400338	5	NULL	NULL	0	NULL	design of experiment ( DOE ) algorithm	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to automate the optimization of complex biochemical and molecular biology reactions , we developed a sequential injection analysis ( SIA ) device and combined this with a design of experiment ( DOE ) algorithm .
	manualset3
100916	1	400339	5	NULL	NULL	0	NULL	vaginal anti-HIV-1 microbicides	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to be effective , the vaginal anti-HIV-1 microbicides should avoid proinflammatory responses that facilitate transepithelial viral penetration and replication .
	manualset3
100917	2	400339	5	NULL	NULL	0	NULL	proinflammatory responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to be effective , the vaginal anti-HIV-1 microbicides should avoid proinflammatory responses that facilitate transepithelial viral penetration and replication .
	manualset3
100918	3	400339	5	NULL	NULL	0	NULL	transepithelial viral penetration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to be effective , the vaginal anti-HIV-1 microbicides should avoid proinflammatory responses that facilitate transepithelial viral penetration and replication .
	manualset3
100920	4	400339	5	NULL	NULL	0	NULL	transepithelial viral replication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to be effective , the vaginal anti-HIV-1 microbicides should avoid proinflammatory responses that facilitate transepithelial viral penetration and replication .
	manualset3
100921	1	400340	5	NULL	NULL	0	NULL	zebrafish embryos	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to clarify this question , we have exposed zebrafish embryos to ethanol and evaluated whether a miRNA deregulation signature could be obtained .
	manualset3
100922	2	400340	5	NULL	NULL	0	NULL	ethanol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to clarify this question , we have exposed zebrafish embryos to ethanol and evaluated whether a miRNA deregulation signature could be obtained .
	manualset3
100923	3	400340	5	NULL	NULL	0	NULL	miRNA deregulation signature	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to clarify this question , we have exposed zebrafish embryos to ethanol and evaluated whether a miRNA deregulation signature could be obtained .
	manualset3
102796	1	400341	5	NULL	NULL	0	NULL	reaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( reaction : see text ) An asymmetric total synthesis of ( - ) - swainsonine and ( + ) -6 - epicastanospermine is described from a common intermediate , which is obtained through diastereoselective ( 2 + 2 ) cycloaddition of dichloroketene to a chiral enol ether .
	manualset3
102797	2	400341	5	NULL	NULL	0	NULL	asymmetric total synthesis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( reaction : see text ) An asymmetric total synthesis of ( - ) - swainsonine and ( + ) -6 - epicastanospermine is described from a common intermediate , which is obtained through diastereoselective ( 2 + 2 ) cycloaddition of dichloroketene to a chiral enol ether .
	manualset3
102798	3	400341	5	NULL	NULL	0	NULL	( - ) - swainsonine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	( reaction : see text ) An asymmetric total synthesis of ( - ) - swainsonine and ( + ) -6 - epicastanospermine is described from a common intermediate , which is obtained through diastereoselective ( 2 + 2 ) cycloaddition of dichloroketene to a chiral enol ether .
	manualset3
102800	4	400341	5	NULL	NULL	0	NULL	( + ) -6 - epicastanospermine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	( reaction : see text ) An asymmetric total synthesis of ( - ) - swainsonine and ( + ) -6 - epicastanospermine is described from a common intermediate , which is obtained through diastereoselective ( 2 + 2 ) cycloaddition of dichloroketene to a chiral enol ether .
	manualset3
102805	5	400341	5	NULL	NULL	0	NULL	intermediate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	( reaction : see text ) An asymmetric total synthesis of ( - ) - swainsonine and ( + ) -6 - epicastanospermine is described from a common intermediate , which is obtained through diastereoselective ( 2 + 2 ) cycloaddition of dichloroketene to a chiral enol ether .
	manualset3
102806	6	400341	5	NULL	NULL	0	NULL	diastereoselective ( 2 + 2 ) cycloaddition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( reaction : see text ) An asymmetric total synthesis of ( - ) - swainsonine and ( + ) -6 - epicastanospermine is described from a common intermediate , which is obtained through diastereoselective ( 2 + 2 ) cycloaddition of dichloroketene to a chiral enol ether .
	manualset3
102807	7	400341	5	NULL	NULL	0	NULL	dichloroketene 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( reaction : see text ) An asymmetric total synthesis of ( - ) - swainsonine and ( + ) -6 - epicastanospermine is described from a common intermediate , which is obtained through diastereoselective ( 2 + 2 ) cycloaddition of dichloroketene to a chiral enol ether .
	manualset3
102808	8	400341	5	NULL	NULL	0	NULL	chiral enol ether 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( reaction : see text ) An asymmetric total synthesis of ( - ) - swainsonine and ( + ) -6 - epicastanospermine is described from a common intermediate , which is obtained through diastereoselective ( 2 + 2 ) cycloaddition of dichloroketene to a chiral enol ether .
	manualset3
100924	1	400342	5	NULL	NULL	0	NULL	biochemical basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to define its biochemical basis , we studied the differential expression of genes involved in hepatic glucose and lipid metabolism by microarray analysis .
	manualset3
100925	2	400342	5	NULL	NULL	0	NULL	differential expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to define its biochemical basis , we studied the differential expression of genes involved in hepatic glucose and lipid metabolism by microarray analysis .
	manualset3
100926	3	400342	5	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to define its biochemical basis , we studied the differential expression of genes involved in hepatic glucose and lipid metabolism by microarray analysis .
	manualset3
100927	4	400342	5	NULL	NULL	0	NULL	hepatic glucose metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to define its biochemical basis , we studied the differential expression of genes involved in hepatic glucose and lipid metabolism by microarray analysis .
	manualset3
100928	5	400342	5	NULL	NULL	0	NULL	hepatic lipid metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to define its biochemical basis , we studied the differential expression of genes involved in hepatic glucose and lipid metabolism by microarray analysis .
	manualset3
100929	6	400342	5	NULL	NULL	0	NULL	microarray analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to define its biochemical basis , we studied the differential expression of genes involved in hepatic glucose and lipid metabolism by microarray analysis .
	manualset3
100930	1	400343	5	NULL	NULL	0	NULL	problem solving skilla	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine change in problem solving and care planning skills we compared ( a ) the previous third year student performance on semester I and II assessments with those of the study participants and ( b ) results at the end of semester I with end of semester II within the study cohort .
	manualset3
100931	2	400343	5	NULL	NULL	0	NULL	care planning skills 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine change in problem solving and care planning skills we compared ( a ) the previous third year student performance on semester I and II assessments with those of the study participants and ( b ) results at the end of semester I with end of semester II within the study cohort .
	manualset3
100932	3	400343	5	NULL	NULL	0	NULL	previous third year student performance	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine change in problem solving and care planning skills we compared ( a ) the previous third year student performance on semester I and II assessments with those of the study participants and ( b ) results at the end of semester I with end of semester II within the study cohort .
	manualset3
100933	4	400343	5	NULL	NULL	0	NULL	semester I and II assessments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine change in problem solving and care planning skills we compared ( a ) the previous third year student performance on semester I and II assessments with those of the study participants and ( b ) results at the end of semester I with end of semester II within the study cohort .
	manualset3
100934	5	400343	5	NULL	NULL	0	NULL	study participants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine change in problem solving and care planning skills we compared ( a ) the previous third year student performance on semester I and II assessments with those of the study participants and ( b ) results at the end of semester I with end of semester II within the study cohort .
	manualset3
100935	6	400343	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine change in problem solving and care planning skills we compared ( a ) the previous third year student performance on semester I and II assessments with those of the study participants and ( b ) results at the end of semester I with end of semester II within the study cohort .
	manualset3
100936	7	400343	5	NULL	NULL	0	NULL	semester I	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine change in problem solving and care planning skills we compared ( a ) the previous third year student performance on semester I and II assessments with those of the study participants and ( b ) results at the end of semester I with end of semester II within the study cohort .
	manualset3
100937	8	400343	5	NULL	NULL	0	NULL	semester II	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine change in problem solving and care planning skills we compared ( a ) the previous third year student performance on semester I and II assessments with those of the study participants and ( b ) results at the end of semester I with end of semester II within the study cohort .
	manualset3
100938	9	400343	5	NULL	NULL	0	NULL	study cohort	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine change in problem solving and care planning skills we compared ( a ) the previous third year student performance on semester I and II assessments with those of the study participants and ( b ) results at the end of semester I with end of semester II within the study cohort .
	manualset3
100939	1	400344	5	NULL	NULL	0	NULL	O-GlcNAc	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine how O-GlcNAc modulates stress tolerance in these models we have used stable isotope labeling with amino acids in cell culture to determine the identity of proteins that undergo O-GlcNAcylation in response to heat shock .
	manualset3
100940	2	400344	5	NULL	NULL	0	NULL	stress tolerance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine how O-GlcNAc modulates stress tolerance in these models we have used stable isotope labeling with amino acids in cell culture to determine the identity of proteins that undergo O-GlcNAcylation in response to heat shock .
	manualset3
100941	3	400344	5	NULL	NULL	0	NULL	models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine how O-GlcNAc modulates stress tolerance in these models we have used stable isotope labeling with amino acids in cell culture to determine the identity of proteins that undergo O-GlcNAcylation in response to heat shock .
	manualset3
100942	4	400344	5	NULL	NULL	0	NULL	stable isotope labeling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine how O-GlcNAc modulates stress tolerance in these models we have used stable isotope labeling with amino acids in cell culture to determine the identity of proteins that undergo O-GlcNAcylation in response to heat shock .
	manualset3
100943	5	400344	5	NULL	NULL	0	NULL	amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine how O-GlcNAc modulates stress tolerance in these models we have used stable isotope labeling with amino acids in cell culture to determine the identity of proteins that undergo O-GlcNAcylation in response to heat shock .
	manualset3
100944	6	400344	5	NULL	NULL	0	NULL	cell culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine how O-GlcNAc modulates stress tolerance in these models we have used stable isotope labeling with amino acids in cell culture to determine the identity of proteins that undergo O-GlcNAcylation in response to heat shock .
	manualset3
100945	7	400344	5	NULL	NULL	0	NULL	proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine how O-GlcNAc modulates stress tolerance in these models we have used stable isotope labeling with amino acids in cell culture to determine the identity of proteins that undergo O-GlcNAcylation in response to heat shock .
	manualset3
100946	8	400344	5	NULL	NULL	0	NULL	O-GlcNAcylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine how O-GlcNAc modulates stress tolerance in these models we have used stable isotope labeling with amino acids in cell culture to determine the identity of proteins that undergo O-GlcNAcylation in response to heat shock .
	manualset3
100947	9	400344	5	NULL	NULL	NULL	NULL	heat shock	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In order to determine how O-GlcNAc modulates stress tolerance in these models we have used stable isotope labeling with amino acids in cell culture to determine the identity of proteins that undergo O-GlcNAcylation in response to heat shock .
	manualset3
100948	1	400345	5	NULL	NULL	0	NULL	cystathionine beta-synthase ( CBS ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine if cystathionine beta-synthase ( CBS ) could separate groups of patients with various vascular disease , CBS activity was studied in cultured human skin fibroblasts from 30 subjects being either controls , atherosclerotic patients or patients having suffered a deep venous thrombosis .
	manualset3
100949	2	400345	5	NULL	NULL	0	NULL	groups of patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine if cystathionine beta-synthase ( CBS ) could separate groups of patients with various vascular disease , CBS activity was studied in cultured human skin fibroblasts from 30 subjects being either controls , atherosclerotic patients or patients having suffered a deep venous thrombosis .
	manualset3
100950	3	400345	5	NULL	NULL	0	NULL	vascular disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine if cystathionine beta-synthase ( CBS ) could separate groups of patients with various vascular disease , CBS activity was studied in cultured human skin fibroblasts from 30 subjects being either controls , atherosclerotic patients or patients having suffered a deep venous thrombosis .
	manualset3
100951	4	400345	5	NULL	NULL	0	NULL	CBS activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine if cystathionine beta-synthase ( CBS ) could separate groups of patients with various vascular disease , CBS activity was studied in cultured human skin fibroblasts from 30 subjects being either controls , atherosclerotic patients or patients having suffered a deep venous thrombosis .
	manualset3
100952	5	400345	5	NULL	NULL	0	NULL	cultured human skin fibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine if cystathionine beta-synthase ( CBS ) could separate groups of patients with various vascular disease , CBS activity was studied in cultured human skin fibroblasts from 30 subjects being either controls , atherosclerotic patients or patients having suffered a deep venous thrombosis .
	manualset3
100953	6	400345	5	NULL	NULL	0	NULL	30 subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine if cystathionine beta-synthase ( CBS ) could separate groups of patients with various vascular disease , CBS activity was studied in cultured human skin fibroblasts from 30 subjects being either controls , atherosclerotic patients or patients having suffered a deep venous thrombosis .
	manualset3
100954	7	400345	5	NULL	NULL	0	NULL	atherosclerotic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine if cystathionine beta-synthase ( CBS ) could separate groups of patients with various vascular disease , CBS activity was studied in cultured human skin fibroblasts from 30 subjects being either controls , atherosclerotic patients or patients having suffered a deep venous thrombosis .
	manualset3
100955	8	400345	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine if cystathionine beta-synthase ( CBS ) could separate groups of patients with various vascular disease , CBS activity was studied in cultured human skin fibroblasts from 30 subjects being either controls , atherosclerotic patients or patients having suffered a deep venous thrombosis .
	manualset3
100956	9	400345	5	NULL	NULL	0	NULL	deep venous thrombosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine if cystathionine beta-synthase ( CBS ) could separate groups of patients with various vascular disease , CBS activity was studied in cultured human skin fibroblasts from 30 subjects being either controls , atherosclerotic patients or patients having suffered a deep venous thrombosis .
	manualset3
100957	1	400346	5	NULL	NULL	0	NULL	small double-membrane-bounded organelle	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine whether the small double-membrane-bounded organelle posterior to the nucleus in the apicomplexan Cryptosporidium parvum is a mitochondrion , the Cpn60 gene of C. parvum sporozoites ( CpCpn60 ) was analyzed and antibodies were generated for localization of the peptide .
	manualset3
100958	2	400346	5	NULL	NULL	0	NULL	nucleus 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine whether the small double-membrane-bounded organelle posterior to the nucleus in the apicomplexan Cryptosporidium parvum is a mitochondrion , the Cpn60 gene of C. parvum sporozoites ( CpCpn60 ) was analyzed and antibodies were generated for localization of the peptide .
	manualset3
100959	3	400346	5	NULL	NULL	0	NULL	apicomplexan Cryptosporidium parvum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine whether the small double-membrane-bounded organelle posterior to the nucleus in the apicomplexan Cryptosporidium parvum is a mitochondrion , the Cpn60 gene of C. parvum sporozoites ( CpCpn60 ) was analyzed and antibodies were generated for localization of the peptide .
	manualset3
100960	4	400346	5	NULL	NULL	0	NULL	mitochondrion	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine whether the small double-membrane-bounded organelle posterior to the nucleus in the apicomplexan Cryptosporidium parvum is a mitochondrion , the Cpn60 gene of C. parvum sporozoites ( CpCpn60 ) was analyzed and antibodies were generated for localization of the peptide .
	manualset3
100961	5	400346	5	NULL	NULL	0	NULL	Cpn60 gene of C. parvum sporozoites ( CpCpn60 )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine whether the small double-membrane-bounded organelle posterior to the nucleus in the apicomplexan Cryptosporidium parvum is a mitochondrion , the Cpn60 gene of C. parvum sporozoites ( CpCpn60 ) was analyzed and antibodies were generated for localization of the peptide .
	manualset3
100962	6	400346	5	NULL	NULL	0	NULL	antibodies 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine whether the small double-membrane-bounded organelle posterior to the nucleus in the apicomplexan Cryptosporidium parvum is a mitochondrion , the Cpn60 gene of C. parvum sporozoites ( CpCpn60 ) was analyzed and antibodies were generated for localization of the peptide .
	manualset3
100963	7	400346	5	NULL	NULL	0	NULL	localization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine whether the small double-membrane-bounded organelle posterior to the nucleus in the apicomplexan Cryptosporidium parvum is a mitochondrion , the Cpn60 gene of C. parvum sporozoites ( CpCpn60 ) was analyzed and antibodies were generated for localization of the peptide .
	manualset3
100964	8	400346	5	NULL	NULL	0	NULL	peptide 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to determine whether the small double-membrane-bounded organelle posterior to the nucleus in the apicomplexan Cryptosporidium parvum is a mitochondrion , the Cpn60 gene of C. parvum sporozoites ( CpCpn60 ) was analyzed and antibodies were generated for localization of the peptide .
	manualset3
100965	1	400347	5	NULL	NULL	0	NULL	treatments 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to develop treatments that improve survival while preserving quality of life for children with brain tumors , a better understanding of brain tumor biology is needed .
	manualset3
100966	2	400347	5	NULL	NULL	0	NULL	survival 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to develop treatments that improve survival while preserving quality of life for children with brain tumors , a better understanding of brain tumor biology is needed .
	manualset3
100967	3	400347	5	NULL	NULL	0	NULL	quality of life	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to develop treatments that improve survival while preserving quality of life for children with brain tumors , a better understanding of brain tumor biology is needed .
	manualset3
100968	4	400347	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to develop treatments that improve survival while preserving quality of life for children with brain tumors , a better understanding of brain tumor biology is needed .
	manualset3
100969	5	400347	5	NULL	NULL	0	NULL	brain tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to develop treatments that improve survival while preserving quality of life for children with brain tumors , a better understanding of brain tumor biology is needed .
	manualset3
100970	6	400347	5	NULL	NULL	0	NULL	brain tumor biology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to develop treatments that improve survival while preserving quality of life for children with brain tumors , a better understanding of brain tumor biology is needed .
	manualset3
100971	1	400348	5	NULL	NULL	0	NULL	bibliography	Citation												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to do this it will lean , on one hand , on the actual bibliography about blood of the umbilical cord and its present and future applications , and on the other hand , on the document of the European Group of Ethics where this issue is discussed .
	manualset3
100972	2	400348	5	NULL	NULL	0	NULL	blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to do this it will lean , on one hand , on the actual bibliography about blood of the umbilical cord and its present and future applications , and on the other hand , on the document of the European Group of Ethics where this issue is discussed .
	manualset3
100973	3	400348	5	NULL	NULL	0	NULL	umbilical cord	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to do this it will lean , on one hand , on the actual bibliography about blood of the umbilical cord and its present and future applications , and on the other hand , on the document of the European Group of Ethics where this issue is discussed .
	manualset3
100974	4	400348	5	NULL	NULL	0	NULL	present applications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to do this it will lean , on one hand , on the actual bibliography about blood of the umbilical cord and its present and future applications , and on the other hand , on the document of the European Group of Ethics where this issue is discussed .
	manualset3
100975	5	400348	5	NULL	NULL	0	NULL	future applications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to do this it will lean , on one hand , on the actual bibliography about blood of the umbilical cord and its present and future applications , and on the other hand , on the document of the European Group of Ethics where this issue is discussed .
	manualset3
100976	6	400348	5	NULL	NULL	0	NULL	document	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to do this it will lean , on one hand , on the actual bibliography about blood of the umbilical cord and its present and future applications , and on the other hand , on the document of the European Group of Ethics where this issue is discussed .
	manualset3
100977	7	400348	5	NULL	NULL	0	NULL	European Group of Ethics	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to do this it will lean , on one hand , on the actual bibliography about blood of the umbilical cord and its present and future applications , and on the other hand , on the document of the European Group of Ethics where this issue is discussed .
	manualset3
100978	8	400348	5	NULL	NULL	0	NULL	issue 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to do this it will lean , on one hand , on the actual bibliography about blood of the umbilical cord and its present and future applications , and on the other hand , on the document of the European Group of Ethics where this issue is discussed .
	manualset3
100979	1	400349	5	NULL	NULL	0	NULL	MPSV 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( v ) MPSV has long terminal repeats and an enhancer sequence more like Mo-MuLV than Mo-MuSV , with a consequently altered target cell specificity .
	manualset3
100980	2	400349	5	NULL	NULL	0	NULL	long terminal repeats	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	( v ) MPSV has long terminal repeats and an enhancer sequence more like Mo-MuLV than Mo-MuSV , with a consequently altered target cell specificity .
	manualset3
100981	3	400349	5	NULL	NULL	0	NULL	enhancer sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	( v ) MPSV has long terminal repeats and an enhancer sequence more like Mo-MuLV than Mo-MuSV , with a consequently altered target cell specificity .
	manualset3
100982	4	400349	5	NULL	NULL	0	NULL	Mo-MuLV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( v ) MPSV has long terminal repeats and an enhancer sequence more like Mo-MuLV than Mo-MuSV , with a consequently altered target cell specificity .
	manualset3
100983	5	400349	5	NULL	NULL	0	NULL	Mo-MuSV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( v ) MPSV has long terminal repeats and an enhancer sequence more like Mo-MuLV than Mo-MuSV , with a consequently altered target cell specificity .
	manualset3
100984	6	400349	5	NULL	NULL	0	NULL	target cell specificity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( v ) MPSV has long terminal repeats and an enhancer sequence more like Mo-MuLV than Mo-MuSV , with a consequently altered target cell specificity .
	manualset3
100985	1	400350	5	NULL	NULL	0	NULL	functionality	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to elucidate the functionality of CsaA further , interaction with its postulated substrate YvaY was investigated .
	manualset3
100986	2	400350	5	NULL	NULL	0	NULL	CsaA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to elucidate the functionality of CsaA further , interaction with its postulated substrate YvaY was investigated .
	manualset3
100987	3	400350	5	NULL	NULL	0	NULL	interaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to elucidate the functionality of CsaA further , interaction with its postulated substrate YvaY was investigated .
	manualset3
100988	4	400350	5	NULL	NULL	0	NULL	postulated substrate YvaY	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to elucidate the functionality of CsaA further , interaction with its postulated substrate YvaY was investigated .
	manualset3
100989	1	400351	5	NULL	NULL	0	NULL	molecular mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to elucidate the molecular mechanism underlying aberrant Pim-3 expression in pancreatic cancer cells , we constructed luciferase expression vectors linked to 5 ' - flanking deletion mutants of the human Pim-3 gene and transfected human pancreatic cancer cells with the resultant vectors .
	manualset3
100990	2	400351	5	NULL	NULL	0	NULL	Pim-3 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to elucidate the molecular mechanism underlying aberrant Pim-3 expression in pancreatic cancer cells , we constructed luciferase expression vectors linked to 5 ' - flanking deletion mutants of the human Pim-3 gene and transfected human pancreatic cancer cells with the resultant vectors .
	manualset3
100991	2	400351	5	NULL	NULL	0	NULL	Pim-3 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to elucidate the molecular mechanism underlying aberrant Pim-3 expression in pancreatic cancer cells , we constructed luciferase expression vectors linked to 5 ' - flanking deletion mutants of the human Pim-3 gene and transfected human pancreatic cancer cells with the resultant vectors .
	manualset3
100992	3	400351	5	NULL	NULL	0	NULL	pancreatic cancer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to elucidate the molecular mechanism underlying aberrant Pim-3 expression in pancreatic cancer cells , we constructed luciferase expression vectors linked to 5 ' - flanking deletion mutants of the human Pim-3 gene and transfected human pancreatic cancer cells with the resultant vectors .
	manualset3
100993	4	400351	5	NULL	NULL	0	NULL	luciferase expression vectors	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to elucidate the molecular mechanism underlying aberrant Pim-3 expression in pancreatic cancer cells , we constructed luciferase expression vectors linked to 5 ' - flanking deletion mutants of the human Pim-3 gene and transfected human pancreatic cancer cells with the resultant vectors .
	manualset3
100994	5	400351	5	NULL	NULL	0	NULL	5 ' - flanking deletion mutants of the human Pim-3 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to elucidate the molecular mechanism underlying aberrant Pim-3 expression in pancreatic cancer cells , we constructed luciferase expression vectors linked to 5 ' - flanking deletion mutants of the human Pim-3 gene and transfected human pancreatic cancer cells with the resultant vectors .
	manualset3
100995	6	400351	5	NULL	NULL	0	NULL	transfected human pancreatic cancer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to elucidate the molecular mechanism underlying aberrant Pim-3 expression in pancreatic cancer cells , we constructed luciferase expression vectors linked to 5 ' - flanking deletion mutants of the human Pim-3 gene and transfected human pancreatic cancer cells with the resultant vectors .
	manualset3
100996	7	400351	5	NULL	NULL	0	NULL	resultant vectors	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to elucidate the molecular mechanism underlying aberrant Pim-3 expression in pancreatic cancer cells , we constructed luciferase expression vectors linked to 5 ' - flanking deletion mutants of the human Pim-3 gene and transfected human pancreatic cancer cells with the resultant vectors .
	manualset3
100997	1	400352	5	NULL	NULL	NULL	NULL	infection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In order to establish a successful infection , Salmonella utilize a large number of genes encoding a variety of virulence factors .
	manualset3
100998	2	400352	5	NULL	NULL	0	NULL	Salmonella 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to establish a successful infection , Salmonella utilize a large number of genes encoding a variety of virulence factors .
	manualset3
100999	3	400352	5	NULL	NULL	0	NULL	large number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to establish a successful infection , Salmonella utilize a large number of genes encoding a variety of virulence factors .
	manualset3
101000	4	400352	5	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to establish a successful infection , Salmonella utilize a large number of genes encoding a variety of virulence factors .
	manualset3
101001	5	400352	5	NULL	NULL	0	NULL	virulence factors	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to establish a successful infection , Salmonella utilize a large number of genes encoding a variety of virulence factors .
	manualset3
101002	1	400353	5	NULL	NULL	0	NULL	involvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to establish the involvement of particular neurochemical brain groups in the response to blood volume expansion , we analyzed Fos-labeling in combination with immunolabeling for serotonin , tyrosine hydroxylase , vasopressin and oxytocin , 90 min after a sham or i.v. isotonic blood volume expansion ( BVE ) in unanesthetized , unrestrained rats .
	manualset3
101003	2	400353	5	NULL	NULL	0	NULL	neurochemical brain groups	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to establish the involvement of particular neurochemical brain groups in the response to blood volume expansion , we analyzed Fos-labeling in combination with immunolabeling for serotonin , tyrosine hydroxylase , vasopressin and oxytocin , 90 min after a sham or i.v. isotonic blood volume expansion ( BVE ) in unanesthetized , unrestrained rats .
	manualset3
101004	3	400353	5	NULL	NULL	0	NULL	blood volume expansion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to establish the involvement of particular neurochemical brain groups in the response to blood volume expansion , we analyzed Fos-labeling in combination with immunolabeling for serotonin , tyrosine hydroxylase , vasopressin and oxytocin , 90 min after a sham or i.v. isotonic blood volume expansion ( BVE ) in unanesthetized , unrestrained rats .
	manualset3
101005	4	400353	5	NULL	NULL	0	NULL	Fos-labeling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to establish the involvement of particular neurochemical brain groups in the response to blood volume expansion , we analyzed Fos-labeling in combination with immunolabeling for serotonin , tyrosine hydroxylase , vasopressin and oxytocin , 90 min after a sham or i.v. isotonic blood volume expansion ( BVE ) in unanesthetized , unrestrained rats .
	manualset3
101006	5	400353	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to establish the involvement of particular neurochemical brain groups in the response to blood volume expansion , we analyzed Fos-labeling in combination with immunolabeling for serotonin , tyrosine hydroxylase , vasopressin and oxytocin , 90 min after a sham or i.v. isotonic blood volume expansion ( BVE ) in unanesthetized , unrestrained rats .
	manualset3
101007	6	400353	5	NULL	NULL	0	NULL	immunolabeling 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to establish the involvement of particular neurochemical brain groups in the response to blood volume expansion , we analyzed Fos-labeling in combination with immunolabeling for serotonin , tyrosine hydroxylase , vasopressin and oxytocin , 90 min after a sham or i.v. isotonic blood volume expansion ( BVE ) in unanesthetized , unrestrained rats .
	manualset3
101008	7	400353	5	NULL	NULL	0	NULL	serotonin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to establish the involvement of particular neurochemical brain groups in the response to blood volume expansion , we analyzed Fos-labeling in combination with immunolabeling for serotonin , tyrosine hydroxylase , vasopressin and oxytocin , 90 min after a sham or i.v. isotonic blood volume expansion ( BVE ) in unanesthetized , unrestrained rats .
	manualset3
101009	8	400353	5	NULL	NULL	0	NULL	tyrosine hydroxylase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to establish the involvement of particular neurochemical brain groups in the response to blood volume expansion , we analyzed Fos-labeling in combination with immunolabeling for serotonin , tyrosine hydroxylase , vasopressin and oxytocin , 90 min after a sham or i.v. isotonic blood volume expansion ( BVE ) in unanesthetized , unrestrained rats .
	manualset3
101010	9	400353	5	NULL	NULL	0	NULL	vasopressin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to establish the involvement of particular neurochemical brain groups in the response to blood volume expansion , we analyzed Fos-labeling in combination with immunolabeling for serotonin , tyrosine hydroxylase , vasopressin and oxytocin , 90 min after a sham or i.v. isotonic blood volume expansion ( BVE ) in unanesthetized , unrestrained rats .
	manualset3
101011	10	400353	5	NULL	NULL	0	NULL	oxytocin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to establish the involvement of particular neurochemical brain groups in the response to blood volume expansion , we analyzed Fos-labeling in combination with immunolabeling for serotonin , tyrosine hydroxylase , vasopressin and oxytocin , 90 min after a sham or i.v. isotonic blood volume expansion ( BVE ) in unanesthetized , unrestrained rats .
	manualset3
101012	11	400353	5	NULL	NULL	0	NULL	90 min	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to establish the involvement of particular neurochemical brain groups in the response to blood volume expansion , we analyzed Fos-labeling in combination with immunolabeling for serotonin , tyrosine hydroxylase , vasopressin and oxytocin , 90 min after a sham or i.v. isotonic blood volume expansion ( BVE ) in unanesthetized , unrestrained rats .
	manualset3
101013	12	400353	5	NULL	NULL	0	NULL	sham 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to establish the involvement of particular neurochemical brain groups in the response to blood volume expansion , we analyzed Fos-labeling in combination with immunolabeling for serotonin , tyrosine hydroxylase , vasopressin and oxytocin , 90 min after a sham or i.v. isotonic blood volume expansion ( BVE ) in unanesthetized , unrestrained rats .
	manualset3
101014	13	400353	5	NULL	NULL	NULL	NULL	i.v. isotonic blood volume expansion ( BVE )	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In order to establish the involvement of particular neurochemical brain groups in the response to blood volume expansion , we analyzed Fos-labeling in combination with immunolabeling for serotonin , tyrosine hydroxylase , vasopressin and oxytocin , 90 min after a sham or i.v. isotonic blood volume expansion ( BVE ) in unanesthetized , unrestrained rats .
	manualset3
101015	14	400353	5	NULL	NULL	0	NULL	unanesthetized , unrestrained rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to establish the involvement of particular neurochemical brain groups in the response to blood volume expansion , we analyzed Fos-labeling in combination with immunolabeling for serotonin , tyrosine hydroxylase , vasopressin and oxytocin , 90 min after a sham or i.v. isotonic blood volume expansion ( BVE ) in unanesthetized , unrestrained rats .
	manualset3
101016	1	400354	5	NULL	NULL	0	NULL	transcripts 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to establish whether these transcripts are functioning in the aged muscle we investigated the expression of bHLH inhibitory factor Id mRNA showing that it does not present significant changes during aging .
	manualset3
101017	2	400354	5	NULL	NULL	0	NULL	aged muscle	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to establish whether these transcripts are functioning in the aged muscle we investigated the expression of bHLH inhibitory factor Id mRNA showing that it does not present significant changes during aging .
	manualset3
101018	3	400354	5	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to establish whether these transcripts are functioning in the aged muscle we investigated the expression of bHLH inhibitory factor Id mRNA showing that it does not present significant changes during aging .
	manualset3
101019	4	400354	5	NULL	NULL	0	NULL	bHLH inhibitory factor Id mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to establish whether these transcripts are functioning in the aged muscle we investigated the expression of bHLH inhibitory factor Id mRNA showing that it does not present significant changes during aging .
	manualset3
101020	5	400354	5	NULL	NULL	0	NULL	significant changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to establish whether these transcripts are functioning in the aged muscle we investigated the expression of bHLH inhibitory factor Id mRNA showing that it does not present significant changes during aging .
	manualset3
101021	6	400354	5	NULL	NULL	0	NULL	aging	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to establish whether these transcripts are functioning in the aged muscle we investigated the expression of bHLH inhibitory factor Id mRNA showing that it does not present significant changes during aging .
	manualset3
101022	1	400355	5	NULL	NULL	0	NULL	effect of interventions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to evaluate the effect of interventions it is necessary to undertake a systematic evaluation of clinical variables : Which variables have the least interobserver error ?
	manualset3
101023	2	400355	5	NULL	NULL	0	NULL	systematic evaluation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to evaluate the effect of interventions it is necessary to undertake a systematic evaluation of clinical variables : Which variables have the least interobserver error ?
	manualset3
101024	3	400355	5	NULL	NULL	0	NULL	clinical variables	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to evaluate the effect of interventions it is necessary to undertake a systematic evaluation of clinical variables : Which variables have the least interobserver error ?
	manualset3
101025	4	400355	5	NULL	NULL	0	NULL	variables 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to evaluate the effect of interventions it is necessary to undertake a systematic evaluation of clinical variables : Which variables have the least interobserver error ?
	manualset3
101026	5	400355	5	NULL	NULL	0	NULL	interobserver error	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to evaluate the effect of interventions it is necessary to undertake a systematic evaluation of clinical variables : Which variables have the least interobserver error ?
	manualset3
101027	1	400356	5	NULL	NULL	0	NULL	examine	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to examine if neurochemical changes are associated with dystonia , KYNA was determined at the age of maximum severity ( 30 days ) and after remission ( 70 days ) .
	manualset3
101028	2	400356	5	NULL	NULL	NULL	NULL	neurochemical changes	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In order to examine if neurochemical changes are associated with dystonia , KYNA was determined at the age of maximum severity ( 30 days ) and after remission ( 70 days ) .
	manualset3
101029	3	400356	5	NULL	NULL	0	NULL	dystonia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to examine if neurochemical changes are associated with dystonia , KYNA was determined at the age of maximum severity ( 30 days ) and after remission ( 70 days ) .
	manualset3
101030	4	400356	5	NULL	NULL	0	NULL	KYNA	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to examine if neurochemical changes are associated with dystonia , KYNA was determined at the age of maximum severity ( 30 days ) and after remission ( 70 days ) .
	manualset3
101031	5	400356	5	NULL	NULL	NULL	NULL	age of maximum severity ( 30 days ) 	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In order to examine if neurochemical changes are associated with dystonia , KYNA was determined at the age of maximum severity ( 30 days ) and after remission ( 70 days ) .
	manualset3
101032	6	400356	5	NULL	NULL	0	NULL	age of maximum severity ( 30 days ) 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to examine if neurochemical changes are associated with dystonia , KYNA was determined at the age of maximum severity ( 30 days ) and after remission ( 70 days ) .
	manualset3
101395	1	400357	5	NULL	NULL	0	NULL	examine	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to examine the possibility of osteopenia , a group of 36 female runners between the ages of 15 and 44 years were evaluated for bone mineral density , menstrual function , and dietary habits .
	manualset3
101396	2	400357	5	NULL	NULL	0	NULL	possibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to examine the possibility of osteopenia , a group of 36 female runners between the ages of 15 and 44 years were evaluated for bone mineral density , menstrual function , and dietary habits .
	manualset3
101397	3	400357	5	NULL	NULL	0	NULL	osteopenia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to examine the possibility of osteopenia , a group of 36 female runners between the ages of 15 and 44 years were evaluated for bone mineral density , menstrual function , and dietary habits .
	manualset3
101398	4	400357	5	NULL	NULL	0	NULL	group of 36 female runners	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to examine the possibility of osteopenia , a group of 36 female runners between the ages of 15 and 44 years were evaluated for bone mineral density , menstrual function , and dietary habits .
	manualset3
101399	5	400357	5	NULL	NULL	0	NULL	ages 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to examine the possibility of osteopenia , a group of 36 female runners between the ages of 15 and 44 years were evaluated for bone mineral density , menstrual function , and dietary habits .
	manualset3
101400	6	400357	5	NULL	NULL	0	NULL	15 years	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to examine the possibility of osteopenia , a group of 36 female runners between the ages of 15 and 44 years were evaluated for bone mineral density , menstrual function , and dietary habits .
	manualset3
101401	7	400357	5	NULL	NULL	0	NULL	44 years	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to examine the possibility of osteopenia , a group of 36 female runners between the ages of 15 and 44 years were evaluated for bone mineral density , menstrual function , and dietary habits .
	manualset3
101402	8	400357	5	NULL	NULL	0	NULL	bone mineral density	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to examine the possibility of osteopenia , a group of 36 female runners between the ages of 15 and 44 years were evaluated for bone mineral density , menstrual function , and dietary habits .
	manualset3
101403	9	400357	5	NULL	NULL	0	NULL	menstrual function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to examine the possibility of osteopenia , a group of 36 female runners between the ages of 15 and 44 years were evaluated for bone mineral density , menstrual function , and dietary habits .
	manualset3
101404	10	400357	5	NULL	NULL	0	NULL	dietary habits	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to examine the possibility of osteopenia , a group of 36 female runners between the ages of 15 and 44 years were evaluated for bone mineral density , menstrual function , and dietary habits .
	manualset3
101405	1	400358	5	NULL	NULL	0	NULL	occurrence of malformed meniscus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to explain the occurrence of malformed meniscus in man , dissections were carried out in various vertebrates ; they revealed that menisci shaped like a plate , disc , or ring are physiological components of the knee joint in several vertebrates .
	manualset3
101406	2	400358	5	NULL	NULL	0	NULL	man 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to explain the occurrence of malformed meniscus in man , dissections were carried out in various vertebrates ; they revealed that menisci shaped like a plate , disc , or ring are physiological components of the knee joint in several vertebrates .
	manualset3
101407	3	400358	5	NULL	NULL	0	NULL	dissections	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to explain the occurrence of malformed meniscus in man , dissections were carried out in various vertebrates ; they revealed that menisci shaped like a plate , disc , or ring are physiological components of the knee joint in several vertebrates .
	manualset3
101408	4	400358	5	NULL	NULL	0	NULL	vertebrates 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to explain the occurrence of malformed meniscus in man , dissections were carried out in various vertebrates ; they revealed that menisci shaped like a plate , disc , or ring are physiological components of the knee joint in several vertebrates .
	manualset3
101409	5	400358	5	NULL	NULL	0	NULL	menisci shaped like a plate , disc , or ring	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to explain the occurrence of malformed meniscus in man , dissections were carried out in various vertebrates ; they revealed that menisci shaped like a plate , disc , or ring are physiological components of the knee joint in several vertebrates .
	manualset3
101410	6	400358	5	NULL	NULL	0	NULL	physiological components	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to explain the occurrence of malformed meniscus in man , dissections were carried out in various vertebrates ; they revealed that menisci shaped like a plate , disc , or ring are physiological components of the knee joint in several vertebrates .
	manualset3
101411	7	400358	5	NULL	NULL	0	NULL	knee joint	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to explain the occurrence of malformed meniscus in man , dissections were carried out in various vertebrates ; they revealed that menisci shaped like a plate , disc , or ring are physiological components of the knee joint in several vertebrates .
	manualset3
101412	8	400358	5	NULL	NULL	0	NULL	vertebrates 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to explain the occurrence of malformed meniscus in man , dissections were carried out in various vertebrates ; they revealed that menisci shaped like a plate , disc , or ring are physiological components of the knee joint in several vertebrates .
	manualset3
101413	1	400359	5	NULL	NULL	0	NULL	causative mutation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to find the causative mutation in this family , direct sequencing of the low density lipoprotein receptor ( LDLR ) gene was performed .
	manualset3
101414	2	400359	5	NULL	NULL	0	NULL	family 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to find the causative mutation in this family , direct sequencing of the low density lipoprotein receptor ( LDLR ) gene was performed .
	manualset3
101415	3	400359	5	NULL	NULL	0	NULL	direct sequencing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to find the causative mutation in this family , direct sequencing of the low density lipoprotein receptor ( LDLR ) gene was performed .
	manualset3
101416	4	400359	5	NULL	NULL	0	NULL	low density lipoprotein receptor ( LDLR ) gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to find the causative mutation in this family , direct sequencing of the low density lipoprotein receptor ( LDLR ) gene was performed .
	manualset3
101417	1	400360	5	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to gain a better understanding of the role of the ICOS co-stimulatory signal in immune responses , we studied the cellular response of T cells to beads coated with anti-ICOS or anti-CD28 , plus sub-optimal anti-CD3 mAb .
	manualset3
101418	2	400360	5	NULL	NULL	0	NULL	ICOS co-stimulatory signal	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to gain a better understanding of the role of the ICOS co-stimulatory signal in immune responses , we studied the cellular response of T cells to beads coated with anti-ICOS or anti-CD28 , plus sub-optimal anti-CD3 mAb .
	manualset3
101419	3	400360	5	NULL	NULL	NULL	NULL	immune responses	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In order to gain a better understanding of the role of the ICOS co-stimulatory signal in immune responses , we studied the cellular response of T cells to beads coated with anti-ICOS or anti-CD28 , plus sub-optimal anti-CD3 mAb .
	manualset3
101420	4	400360	5	NULL	NULL	NULL	NULL	cellular response	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In order to gain a better understanding of the role of the ICOS co-stimulatory signal in immune responses , we studied the cellular response of T cells to beads coated with anti-ICOS or anti-CD28 , plus sub-optimal anti-CD3 mAb .
	manualset3
101421	5	400360	5	NULL	NULL	0	NULL	T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to gain a better understanding of the role of the ICOS co-stimulatory signal in immune responses , we studied the cellular response of T cells to beads coated with anti-ICOS or anti-CD28 , plus sub-optimal anti-CD3 mAb .
	manualset3
101422	6	400360	5	NULL	NULL	0	NULL	beads coated with anti-ICOS	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to gain a better understanding of the role of the ICOS co-stimulatory signal in immune responses , we studied the cellular response of T cells to beads coated with anti-ICOS or anti-CD28 , plus sub-optimal anti-CD3 mAb .
	manualset3
101423	7	400360	5	NULL	NULL	0	NULL	beads coated with anti-CD28	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to gain a better understanding of the role of the ICOS co-stimulatory signal in immune responses , we studied the cellular response of T cells to beads coated with anti-ICOS or anti-CD28 , plus sub-optimal anti-CD3 mAb .
	manualset3
101424	8	400360	5	NULL	NULL	0	NULL	sub-optimal anti-CD3 mAb	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to gain a better understanding of the role of the ICOS co-stimulatory signal in immune responses , we studied the cellular response of T cells to beads coated with anti-ICOS or anti-CD28 , plus sub-optimal anti-CD3 mAb .
	manualset3
101425	1	400361	5	NULL	NULL	0	NULL	high mass yield	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to have a high mass yield and to minimize the energetic cost of the process , the following optimal conditions , 1.5 g of H2SO4 g ( -1 ) of sludge , 700 degrees C and 145 min are more appropriate for use of activated carbon from sludge in water and gas treatments .
	manualset3
101426	2	400361	5	NULL	NULL	0	NULL	energetic cost	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to have a high mass yield and to minimize the energetic cost of the process , the following optimal conditions , 1.5 g of H2SO4 g ( -1 ) of sludge , 700 degrees C and 145 min are more appropriate for use of activated carbon from sludge in water and gas treatments .
	manualset3
101427	3	400361	5	NULL	NULL	0	NULL	process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to have a high mass yield and to minimize the energetic cost of the process , the following optimal conditions , 1.5 g of H2SO4 g ( -1 ) of sludge , 700 degrees C and 145 min are more appropriate for use of activated carbon from sludge in water and gas treatments .
	manualset3
101428	4	400361	5	NULL	NULL	0	NULL	optimal conditions	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to have a high mass yield and to minimize the energetic cost of the process , the following optimal conditions , 1.5 g of H2SO4 g ( -1 ) of sludge , 700 degrees C and 145 min are more appropriate for use of activated carbon from sludge in water and gas treatments .
	manualset3
101429	5	400361	5	NULL	NULL	0	NULL	1.5 g	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to have a high mass yield and to minimize the energetic cost of the process , the following optimal conditions , 1.5 g of H2SO4 g ( -1 ) of sludge , 700 degrees C and 145 min are more appropriate for use of activated carbon from sludge in water and gas treatments .
	manualset3
101430	6	400361	5	NULL	NULL	0	NULL	 H2SO4 g ( -1 ) 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to have a high mass yield and to minimize the energetic cost of the process , the following optimal conditions , 1.5 g of H2SO4 g ( -1 ) of sludge , 700 degrees C and 145 min are more appropriate for use of activated carbon from sludge in water and gas treatments .
	manualset3
101431	7	400361	5	NULL	NULL	0	NULL	sludge	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to have a high mass yield and to minimize the energetic cost of the process , the following optimal conditions , 1.5 g of H2SO4 g ( -1 ) of sludge , 700 degrees C and 145 min are more appropriate for use of activated carbon from sludge in water and gas treatments .
	manualset3
101432	8	400361	5	NULL	NULL	0	NULL	700 degrees C	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to have a high mass yield and to minimize the energetic cost of the process , the following optimal conditions , 1.5 g of H2SO4 g ( -1 ) of sludge , 700 degrees C and 145 min are more appropriate for use of activated carbon from sludge in water and gas treatments .
	manualset3
101433	9	400361	5	NULL	NULL	0	NULL	145 min	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to have a high mass yield and to minimize the energetic cost of the process , the following optimal conditions , 1.5 g of H2SO4 g ( -1 ) of sludge , 700 degrees C and 145 min are more appropriate for use of activated carbon from sludge in water and gas treatments .
	manualset3
101434	10	400361	5	NULL	NULL	0	NULL	activated carbon	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to have a high mass yield and to minimize the energetic cost of the process , the following optimal conditions , 1.5 g of H2SO4 g ( -1 ) of sludge , 700 degrees C and 145 min are more appropriate for use of activated carbon from sludge in water and gas treatments .
	manualset3
101435	11	400361	5	NULL	NULL	0	NULL	sludge	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to have a high mass yield and to minimize the energetic cost of the process , the following optimal conditions , 1.5 g of H2SO4 g ( -1 ) of sludge , 700 degrees C and 145 min are more appropriate for use of activated carbon from sludge in water and gas treatments .
	manualset3
101436	12	400361	5	NULL	NULL	0	NULL	water treatments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to have a high mass yield and to minimize the energetic cost of the process , the following optimal conditions , 1.5 g of H2SO4 g ( -1 ) of sludge , 700 degrees C and 145 min are more appropriate for use of activated carbon from sludge in water and gas treatments .
	manualset3
101437	13	400361	5	NULL	NULL	0	NULL	gas treatments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to have a high mass yield and to minimize the energetic cost of the process , the following optimal conditions , 1.5 g of H2SO4 g ( -1 ) of sludge , 700 degrees C and 145 min are more appropriate for use of activated carbon from sludge in water and gas treatments .
	manualset3
101438	1	400362	5	NULL	NULL	0	NULL	differentially expressed genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to identify genes differentially expressed in leukemia-derived DCs ( AML-DCs ) , a polymerase chain reaction ( PCR ) - based subtraction approach was applied using cDNA from AML-DCs and monocyte-derived DCs from healthy donors as competitors .
	manualset3
101439	2	400362	5	NULL	NULL	0	NULL	leukemia-derived DCs ( AML-DCs )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to identify genes differentially expressed in leukemia-derived DCs ( AML-DCs ) , a polymerase chain reaction ( PCR ) - based subtraction approach was applied using cDNA from AML-DCs and monocyte-derived DCs from healthy donors as competitors .
	manualset3
101440	3	400362	5	NULL	NULL	0	NULL	polymerase chain reaction ( PCR ) - based subtraction approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to identify genes differentially expressed in leukemia-derived DCs ( AML-DCs ) , a polymerase chain reaction ( PCR ) - based subtraction approach was applied using cDNA from AML-DCs and monocyte-derived DCs from healthy donors as competitors .
	manualset3
101441	4	400362	5	NULL	NULL	0	NULL	cDNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to identify genes differentially expressed in leukemia-derived DCs ( AML-DCs ) , a polymerase chain reaction ( PCR ) - based subtraction approach was applied using cDNA from AML-DCs and monocyte-derived DCs from healthy donors as competitors .
	manualset3
101442	5	400362	5	NULL	NULL	0	NULL	AML-DCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to identify genes differentially expressed in leukemia-derived DCs ( AML-DCs ) , a polymerase chain reaction ( PCR ) - based subtraction approach was applied using cDNA from AML-DCs and monocyte-derived DCs from healthy donors as competitors .
	manualset3
101443	6	400362	5	NULL	NULL	0	NULL	monocyte-derived DCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to identify genes differentially expressed in leukemia-derived DCs ( AML-DCs ) , a polymerase chain reaction ( PCR ) - based subtraction approach was applied using cDNA from AML-DCs and monocyte-derived DCs from healthy donors as competitors .
	manualset3
101444	7	400362	5	NULL	NULL	0	NULL	healthy donors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to identify genes differentially expressed in leukemia-derived DCs ( AML-DCs ) , a polymerase chain reaction ( PCR ) - based subtraction approach was applied using cDNA from AML-DCs and monocyte-derived DCs from healthy donors as competitors .
	manualset3
101445	8	400362	5	NULL	NULL	0	NULL	competitors	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to identify genes differentially expressed in leukemia-derived DCs ( AML-DCs ) , a polymerase chain reaction ( PCR ) - based subtraction approach was applied using cDNA from AML-DCs and monocyte-derived DCs from healthy donors as competitors .
	manualset3
101446	1	400363	5	NULL	NULL	NULL	NULL	wide relevance	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In order to illustrate the wide relevance of the approach , we discuss how it can facilitate research at all levels of PHC : i.e. , in relation to aspects of medical practice ( the case of medically unexplained symptoms ) ; shifts in service organization ( changing professional roles and the introduction of policy reforms ) ; and issues which straddle both organization and content ( the increasing use of complementary medicine in primary care ) .
	manualset3
101447	2	400363	5	NULL	NULL	NULL	NULL	research 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In order to illustrate the wide relevance of the approach , we discuss how it can facilitate research at all levels of PHC : i.e. , in relation to aspects of medical practice ( the case of medically unexplained symptoms ) ; shifts in service organization ( changing professional roles and the introduction of policy reforms ) ; and issues which straddle both organization and content ( the increasing use of complementary medicine in primary care ) .
	manualset3
101448	3	400363	5	NULL	NULL	0	NULL	levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to illustrate the wide relevance of the approach , we discuss how it can facilitate research at all levels of PHC : i.e. , in relation to aspects of medical practice ( the case of medically unexplained symptoms ) ; shifts in service organization ( changing professional roles and the introduction of policy reforms ) ; and issues which straddle both organization and content ( the increasing use of complementary medicine in primary care ) .
	manualset3
101449	4	400363	5	NULL	NULL	0	NULL	PHC	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to illustrate the wide relevance of the approach , we discuss how it can facilitate research at all levels of PHC : i.e. , in relation to aspects of medical practice ( the case of medically unexplained symptoms ) ; shifts in service organization ( changing professional roles and the introduction of policy reforms ) ; and issues which straddle both organization and content ( the increasing use of complementary medicine in primary care ) .
	manualset3
101450	5	400363	5	NULL	NULL	0	NULL	relation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to illustrate the wide relevance of the approach , we discuss how it can facilitate research at all levels of PHC : i.e. , in relation to aspects of medical practice ( the case of medically unexplained symptoms ) ; shifts in service organization ( changing professional roles and the introduction of policy reforms ) ; and issues which straddle both organization and content ( the increasing use of complementary medicine in primary care ) .
	manualset3
101451	6	400363	5	NULL	NULL	0	NULL	 aspects of medical practice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to illustrate the wide relevance of the approach , we discuss how it can facilitate research at all levels of PHC : i.e. , in relation to aspects of medical practice ( the case of medically unexplained symptoms ) ; shifts in service organization ( changing professional roles and the introduction of policy reforms ) ; and issues which straddle both organization and content ( the increasing use of complementary medicine in primary care ) .
	manualset3
101452	7	400363	5	NULL	NULL	NULL	NULL	case	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In order to illustrate the wide relevance of the approach , we discuss how it can facilitate research at all levels of PHC : i.e. , in relation to aspects of medical practice ( the case of medically unexplained symptoms ) ; shifts in service organization ( changing professional roles and the introduction of policy reforms ) ; and issues which straddle both organization and content ( the increasing use of complementary medicine in primary care ) .
	manualset3
101453	8	400363	5	NULL	NULL	0	NULL	medically unexplained symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to illustrate the wide relevance of the approach , we discuss how it can facilitate research at all levels of PHC : i.e. , in relation to aspects of medical practice ( the case of medically unexplained symptoms ) ; shifts in service organization ( changing professional roles and the introduction of policy reforms ) ; and issues which straddle both organization and content ( the increasing use of complementary medicine in primary care ) .
	manualset3
101454	9	400363	5	NULL	NULL	0	NULL	shifts 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to illustrate the wide relevance of the approach , we discuss how it can facilitate research at all levels of PHC : i.e. , in relation to aspects of medical practice ( the case of medically unexplained symptoms ) ; shifts in service organization ( changing professional roles and the introduction of policy reforms ) ; and issues which straddle both organization and content ( the increasing use of complementary medicine in primary care ) .
	manualset3
101455	10	400363	5	NULL	NULL	0	NULL	service organization	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to illustrate the wide relevance of the approach , we discuss how it can facilitate research at all levels of PHC : i.e. , in relation to aspects of medical practice ( the case of medically unexplained symptoms ) ; shifts in service organization ( changing professional roles and the introduction of policy reforms ) ; and issues which straddle both organization and content ( the increasing use of complementary medicine in primary care ) .
	manualset3
101456	11	400363	5	NULL	NULL	0	NULL	professional roles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to illustrate the wide relevance of the approach , we discuss how it can facilitate research at all levels of PHC : i.e. , in relation to aspects of medical practice ( the case of medically unexplained symptoms ) ; shifts in service organization ( changing professional roles and the introduction of policy reforms ) ; and issues which straddle both organization and content ( the increasing use of complementary medicine in primary care ) .
	manualset3
101457	12	400363	5	NULL	NULL	0	NULL	introduction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to illustrate the wide relevance of the approach , we discuss how it can facilitate research at all levels of PHC : i.e. , in relation to aspects of medical practice ( the case of medically unexplained symptoms ) ; shifts in service organization ( changing professional roles and the introduction of policy reforms ) ; and issues which straddle both organization and content ( the increasing use of complementary medicine in primary care ) .
	manualset3
101458	13	400363	5	NULL	NULL	0	NULL	policy reforms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to illustrate the wide relevance of the approach , we discuss how it can facilitate research at all levels of PHC : i.e. , in relation to aspects of medical practice ( the case of medically unexplained symptoms ) ; shifts in service organization ( changing professional roles and the introduction of policy reforms ) ; and issues which straddle both organization and content ( the increasing use of complementary medicine in primary care ) .
	manualset3
101459	14	400363	5	NULL	NULL	0	NULL	issues	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to illustrate the wide relevance of the approach , we discuss how it can facilitate research at all levels of PHC : i.e. , in relation to aspects of medical practice ( the case of medically unexplained symptoms ) ; shifts in service organization ( changing professional roles and the introduction of policy reforms ) ; and issues which straddle both organization and content ( the increasing use of complementary medicine in primary care ) .
	manualset3
101460	15	400363	5	NULL	NULL	0	NULL	organization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to illustrate the wide relevance of the approach , we discuss how it can facilitate research at all levels of PHC : i.e. , in relation to aspects of medical practice ( the case of medically unexplained symptoms ) ; shifts in service organization ( changing professional roles and the introduction of policy reforms ) ; and issues which straddle both organization and content ( the increasing use of complementary medicine in primary care ) .
	manualset3
101461	16	400363	5	NULL	NULL	0	NULL	content 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to illustrate the wide relevance of the approach , we discuss how it can facilitate research at all levels of PHC : i.e. , in relation to aspects of medical practice ( the case of medically unexplained symptoms ) ; shifts in service organization ( changing professional roles and the introduction of policy reforms ) ; and issues which straddle both organization and content ( the increasing use of complementary medicine in primary care ) .
	manualset3
101462	17	400363	5	NULL	NULL	0	NULL	use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to illustrate the wide relevance of the approach , we discuss how it can facilitate research at all levels of PHC : i.e. , in relation to aspects of medical practice ( the case of medically unexplained symptoms ) ; shifts in service organization ( changing professional roles and the introduction of policy reforms ) ; and issues which straddle both organization and content ( the increasing use of complementary medicine in primary care ) .
	manualset3
101463	18	400363	5	NULL	NULL	NULL	NULL	complementary medicine	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In order to illustrate the wide relevance of the approach , we discuss how it can facilitate research at all levels of PHC : i.e. , in relation to aspects of medical practice ( the case of medically unexplained symptoms ) ; shifts in service organization ( changing professional roles and the introduction of policy reforms ) ; and issues which straddle both organization and content ( the increasing use of complementary medicine in primary care ) .
	manualset3
101464	19	400363	5	NULL	NULL	0	NULL	primary care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to illustrate the wide relevance of the approach , we discuss how it can facilitate research at all levels of PHC : i.e. , in relation to aspects of medical practice ( the case of medically unexplained symptoms ) ; shifts in service organization ( changing professional roles and the introduction of policy reforms ) ; and issues which straddle both organization and content ( the increasing use of complementary medicine in primary care ) .
	manualset3
101465	1	400364	5	NULL	NULL	0	NULL	properties 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to improve the properties of FA/cement mixtures , the use of additives was tested .
	manualset3
101466	2	400364	5	NULL	NULL	0	NULL	FA/cement mixtures	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to improve the properties of FA/cement mixtures , the use of additives was tested .
	manualset3
101467	3	400364	5	NULL	NULL	0	NULL	additives 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to improve the properties of FA/cement mixtures , the use of additives was tested .
	manualset3
101468	1	400365	5	NULL	NULL	0	NULL	investigate 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to investigate this interaction , we generated a recombinant baculovirus for the expression of beta-arrestin in Sf9 insect cells .
	manualset3
101469	2	400365	5	NULL	NULL	0	NULL	interaction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to investigate this interaction , we generated a recombinant baculovirus for the expression of beta-arrestin in Sf9 insect cells .
	manualset3
101470	3	400365	5	NULL	NULL	0	NULL	recombinant baculovirus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to investigate this interaction , we generated a recombinant baculovirus for the expression of beta-arrestin in Sf9 insect cells .
	manualset3
101471	4	400365	5	NULL	NULL	NULL	NULL	expression 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In order to investigate this interaction , we generated a recombinant baculovirus for the expression of beta-arrestin in Sf9 insect cells .
	manualset3
101472	5	400365	5	NULL	NULL	NULL	NULL	beta-arrestin	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In order to investigate this interaction , we generated a recombinant baculovirus for the expression of beta-arrestin in Sf9 insect cells .
	manualset3
101473	6	400365	5	NULL	NULL	0	NULL	Sf9 insect cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to investigate this interaction , we generated a recombinant baculovirus for the expression of beta-arrestin in Sf9 insect cells .
	manualset3
101474	1	400366	5	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to know the role of the insulin receptor internalization in the inhibiting effect of B-IgG , we employed CHO cells expressing mutant insulin receptors which do not undergo internalization ( CHO-K1018R ) .
	manualset3
101475	2	400366	5	NULL	NULL	0	NULL	insulin receptor internalization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to know the role of the insulin receptor internalization in the inhibiting effect of B-IgG , we employed CHO cells expressing mutant insulin receptors which do not undergo internalization ( CHO-K1018R ) .
	manualset3
101476	3	400366	5	NULL	NULL	0	NULL	inhibiting effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to know the role of the insulin receptor internalization in the inhibiting effect of B-IgG , we employed CHO cells expressing mutant insulin receptors which do not undergo internalization ( CHO-K1018R ) .
	manualset3
101477	4	400366	5	NULL	NULL	0	NULL	B-IgG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to know the role of the insulin receptor internalization in the inhibiting effect of B-IgG , we employed CHO cells expressing mutant insulin receptors which do not undergo internalization ( CHO-K1018R ) .
	manualset3
101478	5	400366	5	NULL	NULL	0	NULL	CHO cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to know the role of the insulin receptor internalization in the inhibiting effect of B-IgG , we employed CHO cells expressing mutant insulin receptors which do not undergo internalization ( CHO-K1018R ) .
	manualset3
101479	6	400366	5	NULL	NULL	0	NULL	mutant insulin receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to know the role of the insulin receptor internalization in the inhibiting effect of B-IgG , we employed CHO cells expressing mutant insulin receptors which do not undergo internalization ( CHO-K1018R ) .
	manualset3
101480	7	400366	5	NULL	NULL	0	NULL	internalization 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to know the role of the insulin receptor internalization in the inhibiting effect of B-IgG , we employed CHO cells expressing mutant insulin receptors which do not undergo internalization ( CHO-K1018R ) .
	manualset3
101481	8	400366	5	NULL	NULL	0	NULL	( CHO-K1018R )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to know the role of the insulin receptor internalization in the inhibiting effect of B-IgG , we employed CHO cells expressing mutant insulin receptors which do not undergo internalization ( CHO-K1018R ) .
	manualset3
101482	1	400367	5	NULL	NULL	0	NULL	retention times	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to predict retention times for temperature gradients with different start temperatures in LC , another relationship is required to describe the influence of temperature on retention .
	manualset3
101483	2	400367	5	NULL	NULL	0	NULL	temperature gradients	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to predict retention times for temperature gradients with different start temperatures in LC , another relationship is required to describe the influence of temperature on retention .
	manualset3
101484	3	400367	5	NULL	NULL	0	NULL	start temperatures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to predict retention times for temperature gradients with different start temperatures in LC , another relationship is required to describe the influence of temperature on retention .
	manualset3
101485	4	400367	5	NULL	NULL	0	NULL	LC	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to predict retention times for temperature gradients with different start temperatures in LC , another relationship is required to describe the influence of temperature on retention .
	manualset3
101486	5	400367	5	NULL	NULL	0	NULL	relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to predict retention times for temperature gradients with different start temperatures in LC , another relationship is required to describe the influence of temperature on retention .
	manualset3
101487	6	400367	5	NULL	NULL	0	NULL	influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to predict retention times for temperature gradients with different start temperatures in LC , another relationship is required to describe the influence of temperature on retention .
	manualset3
101488	7	400367	5	NULL	NULL	0	NULL	temperature	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to predict retention times for temperature gradients with different start temperatures in LC , another relationship is required to describe the influence of temperature on retention .
	manualset3
101489	8	400367	5	NULL	NULL	0	NULL	retention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to predict retention times for temperature gradients with different start temperatures in LC , another relationship is required to describe the influence of temperature on retention .
	manualset3
101490	1	400368	5	NULL	NULL	0	NULL	framework	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to provide a framework for reviewing the voluminous literature on unemployment and suicidal behavior , the author distinguishes between two categories of deliberately self-harmful act : those with fatal outcome ( suicide ) and those with non-fatal outcome ( parasuicide ) ; and differentiates four major types of quantitative research report : individual -- cross-sectional ; aggregate -- cross-sectional ; individual -- longitudinal ; and aggregate -- longitudinal .
	manualset3
101491	2	400368	5	NULL	NULL	0	NULL	voluminous literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to provide a framework for reviewing the voluminous literature on unemployment and suicidal behavior , the author distinguishes between two categories of deliberately self-harmful act : those with fatal outcome ( suicide ) and those with non-fatal outcome ( parasuicide ) ; and differentiates four major types of quantitative research report : individual -- cross-sectional ; aggregate -- cross-sectional ; individual -- longitudinal ; and aggregate -- longitudinal .
	manualset3
101492	3	400368	5	NULL	NULL	0	NULL	unemployment 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to provide a framework for reviewing the voluminous literature on unemployment and suicidal behavior , the author distinguishes between two categories of deliberately self-harmful act : those with fatal outcome ( suicide ) and those with non-fatal outcome ( parasuicide ) ; and differentiates four major types of quantitative research report : individual -- cross-sectional ; aggregate -- cross-sectional ; individual -- longitudinal ; and aggregate -- longitudinal .
	manualset3
101493	4	400368	5	NULL	NULL	NULL	NULL	suicidal behavior	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In order to provide a framework for reviewing the voluminous literature on unemployment and suicidal behavior , the author distinguishes between two categories of deliberately self-harmful act : those with fatal outcome ( suicide ) and those with non-fatal outcome ( parasuicide ) ; and differentiates four major types of quantitative research report : individual -- cross-sectional ; aggregate -- cross-sectional ; individual -- longitudinal ; and aggregate -- longitudinal .
	manualset3
101494	5	400368	5	NULL	NULL	0	NULL	author	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to provide a framework for reviewing the voluminous literature on unemployment and suicidal behavior , the author distinguishes between two categories of deliberately self-harmful act : those with fatal outcome ( suicide ) and those with non-fatal outcome ( parasuicide ) ; and differentiates four major types of quantitative research report : individual -- cross-sectional ; aggregate -- cross-sectional ; individual -- longitudinal ; and aggregate -- longitudinal .
	manualset3
101495	6	400368	5	NULL	NULL	0	NULL	two categories	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to provide a framework for reviewing the voluminous literature on unemployment and suicidal behavior , the author distinguishes between two categories of deliberately self-harmful act : those with fatal outcome ( suicide ) and those with non-fatal outcome ( parasuicide ) ; and differentiates four major types of quantitative research report : individual -- cross-sectional ; aggregate -- cross-sectional ; individual -- longitudinal ; and aggregate -- longitudinal .
	manualset3
101496	7	400368	5	NULL	NULL	0	NULL	deliberately self-harmful act 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to provide a framework for reviewing the voluminous literature on unemployment and suicidal behavior , the author distinguishes between two categories of deliberately self-harmful act : those with fatal outcome ( suicide ) and those with non-fatal outcome ( parasuicide ) ; and differentiates four major types of quantitative research report : individual -- cross-sectional ; aggregate -- cross-sectional ; individual -- longitudinal ; and aggregate -- longitudinal .
	manualset3
101497	8	400368	5	NULL	NULL	0	NULL	fatal outcome ( suicide ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to provide a framework for reviewing the voluminous literature on unemployment and suicidal behavior , the author distinguishes between two categories of deliberately self-harmful act : those with fatal outcome ( suicide ) and those with non-fatal outcome ( parasuicide ) ; and differentiates four major types of quantitative research report : individual -- cross-sectional ; aggregate -- cross-sectional ; individual -- longitudinal ; and aggregate -- longitudinal .
	manualset3
101498	9	400368	5	NULL	NULL	0	NULL	non-fatal outcome ( parasuicide )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to provide a framework for reviewing the voluminous literature on unemployment and suicidal behavior , the author distinguishes between two categories of deliberately self-harmful act : those with fatal outcome ( suicide ) and those with non-fatal outcome ( parasuicide ) ; and differentiates four major types of quantitative research report : individual -- cross-sectional ; aggregate -- cross-sectional ; individual -- longitudinal ; and aggregate -- longitudinal .
	manualset3
101499	10	400368	5	NULL	NULL	0	NULL	types of quantitative research report 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to provide a framework for reviewing the voluminous literature on unemployment and suicidal behavior , the author distinguishes between two categories of deliberately self-harmful act : those with fatal outcome ( suicide ) and those with non-fatal outcome ( parasuicide ) ; and differentiates four major types of quantitative research report : individual -- cross-sectional ; aggregate -- cross-sectional ; individual -- longitudinal ; and aggregate -- longitudinal .
	manualset3
101500	1	400369	5	NULL	NULL	NULL	NULL	proof of patient information	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In order to provide proof of patient information , the practitioner usually required the patient 's signature ( 58.3 % of cases ) ; less commonly , the referring physician was informed by letter ( 13.9 % of cases ) or a note was made in the patient 's file ( 33.9 % of cases ) .
	manualset3
101501	2	400369	5	NULL	NULL	0	NULL	practitioner	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to provide proof of patient information , the practitioner usually required the patient 's signature ( 58.3 % of cases ) ; less commonly , the referring physician was informed by letter ( 13.9 % of cases ) or a note was made in the patient 's file ( 33.9 % of cases ) .
	manualset3
101502	3	400369	5	NULL	NULL	0	NULL	patient 's signature	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to provide proof of patient information , the practitioner usually required the patient 's signature ( 58.3 % of cases ) ; less commonly , the referring physician was informed by letter ( 13.9 % of cases ) or a note was made in the patient 's file ( 33.9 % of cases ) .
	manualset3
101503	4	400369	5	NULL	NULL	0	NULL	58.3 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to provide proof of patient information , the practitioner usually required the patient 's signature ( 58.3 % of cases ) ; less commonly , the referring physician was informed by letter ( 13.9 % of cases ) or a note was made in the patient 's file ( 33.9 % of cases ) .
	manualset3
101504	5	400369	5	NULL	NULL	0	NULL	cases	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to provide proof of patient information , the practitioner usually required the patient 's signature ( 58.3 % of cases ) ; less commonly , the referring physician was informed by letter ( 13.9 % of cases ) or a note was made in the patient 's file ( 33.9 % of cases ) .
	manualset3
101505	6	400369	5	NULL	NULL	0	NULL	referring physician	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to provide proof of patient information , the practitioner usually required the patient 's signature ( 58.3 % of cases ) ; less commonly , the referring physician was informed by letter ( 13.9 % of cases ) or a note was made in the patient 's file ( 33.9 % of cases ) .
	manualset3
101506	7	400369	5	NULL	NULL	0	NULL	letter	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to provide proof of patient information , the practitioner usually required the patient 's signature ( 58.3 % of cases ) ; less commonly , the referring physician was informed by letter ( 13.9 % of cases ) or a note was made in the patient 's file ( 33.9 % of cases ) .
	manualset3
101507	8	400369	5	NULL	NULL	0	NULL	13.9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to provide proof of patient information , the practitioner usually required the patient 's signature ( 58.3 % of cases ) ; less commonly , the referring physician was informed by letter ( 13.9 % of cases ) or a note was made in the patient 's file ( 33.9 % of cases ) .
	manualset3
101508	9	400369	5	NULL	NULL	0	NULL	cases	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to provide proof of patient information , the practitioner usually required the patient 's signature ( 58.3 % of cases ) ; less commonly , the referring physician was informed by letter ( 13.9 % of cases ) or a note was made in the patient 's file ( 33.9 % of cases ) .
	manualset3
101509	10	400369	5	NULL	NULL	0	NULL	note	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to provide proof of patient information , the practitioner usually required the patient 's signature ( 58.3 % of cases ) ; less commonly , the referring physician was informed by letter ( 13.9 % of cases ) or a note was made in the patient 's file ( 33.9 % of cases ) .
	manualset3
101510	11	400369	5	NULL	NULL	0	NULL	patient 's file	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to provide proof of patient information , the practitioner usually required the patient 's signature ( 58.3 % of cases ) ; less commonly , the referring physician was informed by letter ( 13.9 % of cases ) or a note was made in the patient 's file ( 33.9 % of cases ) .
	manualset3
101511	12	400369	5	NULL	NULL	0	NULL	33.9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to provide proof of patient information , the practitioner usually required the patient 's signature ( 58.3 % of cases ) ; less commonly , the referring physician was informed by letter ( 13.9 % of cases ) or a note was made in the patient 's file ( 33.9 % of cases ) .
	manualset3
101512	13	400369	5	NULL	NULL	0	NULL	cases	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to provide proof of patient information , the practitioner usually required the patient 's signature ( 58.3 % of cases ) ; less commonly , the referring physician was informed by letter ( 13.9 % of cases ) or a note was made in the patient 's file ( 33.9 % of cases ) .
	manualset3
101513	1	400370	5	NULL	NULL	0	NULL	 spatial distribution characteristics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to reveal spatial distribution characteristics of nutrient in the surface sediments of Lake Changshouhu , contents of total nitrogen ( TN ) , total phosphorus ( TP ) and organic matter ( OM ) of 62 surface sediments samples were determined and compared with other urban ( suburban ) lakes in China .
	manualset3
101514	2	400370	5	NULL	NULL	0	NULL	nutrient	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to reveal spatial distribution characteristics of nutrient in the surface sediments of Lake Changshouhu , contents of total nitrogen ( TN ) , total phosphorus ( TP ) and organic matter ( OM ) of 62 surface sediments samples were determined and compared with other urban ( suburban ) lakes in China .
	manualset3
101515	3	400370	5	NULL	NULL	0	NULL	 surface sediments	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to reveal spatial distribution characteristics of nutrient in the surface sediments of Lake Changshouhu , contents of total nitrogen ( TN ) , total phosphorus ( TP ) and organic matter ( OM ) of 62 surface sediments samples were determined and compared with other urban ( suburban ) lakes in China .
	manualset3
101516	4	400370	5	NULL	NULL	0	NULL	Lake Changshouhu	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to reveal spatial distribution characteristics of nutrient in the surface sediments of Lake Changshouhu , contents of total nitrogen ( TN ) , total phosphorus ( TP ) and organic matter ( OM ) of 62 surface sediments samples were determined and compared with other urban ( suburban ) lakes in China .
	manualset3
101517	5	400370	5	NULL	NULL	0	NULL	contents 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to reveal spatial distribution characteristics of nutrient in the surface sediments of Lake Changshouhu , contents of total nitrogen ( TN ) , total phosphorus ( TP ) and organic matter ( OM ) of 62 surface sediments samples were determined and compared with other urban ( suburban ) lakes in China .
	manualset3
101518	6	400370	5	NULL	NULL	0	NULL	total nitrogen ( TN )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to reveal spatial distribution characteristics of nutrient in the surface sediments of Lake Changshouhu , contents of total nitrogen ( TN ) , total phosphorus ( TP ) and organic matter ( OM ) of 62 surface sediments samples were determined and compared with other urban ( suburban ) lakes in China .
	manualset3
101519	7	400370	5	NULL	NULL	0	NULL	total phosphorus ( TP )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to reveal spatial distribution characteristics of nutrient in the surface sediments of Lake Changshouhu , contents of total nitrogen ( TN ) , total phosphorus ( TP ) and organic matter ( OM ) of 62 surface sediments samples were determined and compared with other urban ( suburban ) lakes in China .
	manualset3
101520	8	400370	5	NULL	NULL	0	NULL	organic matter ( OM )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to reveal spatial distribution characteristics of nutrient in the surface sediments of Lake Changshouhu , contents of total nitrogen ( TN ) , total phosphorus ( TP ) and organic matter ( OM ) of 62 surface sediments samples were determined and compared with other urban ( suburban ) lakes in China .
	manualset3
101521	9	400370	5	NULL	NULL	0	NULL	62 surface sediments samples	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to reveal spatial distribution characteristics of nutrient in the surface sediments of Lake Changshouhu , contents of total nitrogen ( TN ) , total phosphorus ( TP ) and organic matter ( OM ) of 62 surface sediments samples were determined and compared with other urban ( suburban ) lakes in China .
	manualset3
101522	10	400370	5	NULL	NULL	NULL	NULL	urban ( suburban ) lakes	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In order to reveal spatial distribution characteristics of nutrient in the surface sediments of Lake Changshouhu , contents of total nitrogen ( TN ) , total phosphorus ( TP ) and organic matter ( OM ) of 62 surface sediments samples were determined and compared with other urban ( suburban ) lakes in China .
	manualset3
101523	11	400370	5	NULL	NULL	0	NULL	China	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to reveal spatial distribution characteristics of nutrient in the surface sediments of Lake Changshouhu , contents of total nitrogen ( TN ) , total phosphorus ( TP ) and organic matter ( OM ) of 62 surface sediments samples were determined and compared with other urban ( suburban ) lakes in China .
	manualset3
101524	1	400371	5	NULL	NULL	0	NULL	hydroxyl groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to see whether the hydroxyl groups of the sugar parts in the ligand are necessary for the adsorption of the enzyme , chromatography was performed by using the adsorbents prepared with sugar derivatives as the ligand .
	manualset3
101525	2	400371	5	NULL	NULL	0	NULL	sugar parts in the ligand	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to see whether the hydroxyl groups of the sugar parts in the ligand are necessary for the adsorption of the enzyme , chromatography was performed by using the adsorbents prepared with sugar derivatives as the ligand .
	manualset3
101526	3	400371	5	NULL	NULL	0	NULL	adsorption 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to see whether the hydroxyl groups of the sugar parts in the ligand are necessary for the adsorption of the enzyme , chromatography was performed by using the adsorbents prepared with sugar derivatives as the ligand .
	manualset3
101527	4	400371	5	NULL	NULL	0	NULL	enzyme 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to see whether the hydroxyl groups of the sugar parts in the ligand are necessary for the adsorption of the enzyme , chromatography was performed by using the adsorbents prepared with sugar derivatives as the ligand .
	manualset3
101528	5	400371	5	NULL	NULL	0	NULL	chromatography 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to see whether the hydroxyl groups of the sugar parts in the ligand are necessary for the adsorption of the enzyme , chromatography was performed by using the adsorbents prepared with sugar derivatives as the ligand .
	manualset3
101529	6	400371	5	NULL	NULL	0	NULL	adsorbents 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to see whether the hydroxyl groups of the sugar parts in the ligand are necessary for the adsorption of the enzyme , chromatography was performed by using the adsorbents prepared with sugar derivatives as the ligand .
	manualset3
101530	7	400371	5	NULL	NULL	0	NULL	sugar derivatives	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to see whether the hydroxyl groups of the sugar parts in the ligand are necessary for the adsorption of the enzyme , chromatography was performed by using the adsorbents prepared with sugar derivatives as the ligand .
	manualset3
101531	8	400371	5	NULL	NULL	0	NULL	ligand	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to see whether the hydroxyl groups of the sugar parts in the ligand are necessary for the adsorption of the enzyme , chromatography was performed by using the adsorbents prepared with sugar derivatives as the ligand .
	manualset3
101532	1	400372	5	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to study cognitive deficit and the presence of signs and symptoms of depression , 62 elderly community subjects enrolled at a Community Health Unit in Porto Alegre , southern Brazil , were interviewed .
	manualset3
101533	2	400372	5	NULL	NULL	0	NULL	cognitive deficit	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to study cognitive deficit and the presence of signs and symptoms of depression , 62 elderly community subjects enrolled at a Community Health Unit in Porto Alegre , southern Brazil , were interviewed .
	manualset3
101534	3	400372	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to study cognitive deficit and the presence of signs and symptoms of depression , 62 elderly community subjects enrolled at a Community Health Unit in Porto Alegre , southern Brazil , were interviewed .
	manualset3
101535	4	400372	5	NULL	NULL	0	NULL	signs of depression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to study cognitive deficit and the presence of signs and symptoms of depression , 62 elderly community subjects enrolled at a Community Health Unit in Porto Alegre , southern Brazil , were interviewed .
	manualset3
101536	5	400372	5	NULL	NULL	0	NULL	symptoms of depression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to study cognitive deficit and the presence of signs and symptoms of depression , 62 elderly community subjects enrolled at a Community Health Unit in Porto Alegre , southern Brazil , were interviewed .
	manualset3
101537	6	400372	5	NULL	NULL	0	NULL	62 elderly community subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to study cognitive deficit and the presence of signs and symptoms of depression , 62 elderly community subjects enrolled at a Community Health Unit in Porto Alegre , southern Brazil , were interviewed .
	manualset3
101538	7	400372	5	NULL	NULL	0	NULL	Community Health Unit	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to study cognitive deficit and the presence of signs and symptoms of depression , 62 elderly community subjects enrolled at a Community Health Unit in Porto Alegre , southern Brazil , were interviewed .
	manualset3
101539	8	400372	5	NULL	NULL	0	NULL	Porto Alegre , southern Brazil 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to study cognitive deficit and the presence of signs and symptoms of depression , 62 elderly community subjects enrolled at a Community Health Unit in Porto Alegre , southern Brazil , were interviewed .
	manualset3
101540	1	400373	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to study individual differences in response to the genotoxicity of diepoxybutane , we devised a human lymphocyte culture system that involves short-term culture of T lymphocytes and measurement of sister chromatid exchange ( SCE ) and chromosomal aberration frequency as genotoxic end-points .
	manualset3
101541	2	400373	5	NULL	NULL	0	NULL	individual differences	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to study individual differences in response to the genotoxicity of diepoxybutane , we devised a human lymphocyte culture system that involves short-term culture of T lymphocytes and measurement of sister chromatid exchange ( SCE ) and chromosomal aberration frequency as genotoxic end-points .
	manualset3
101542	3	400373	5	NULL	NULL	0	NULL	response	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to study individual differences in response to the genotoxicity of diepoxybutane , we devised a human lymphocyte culture system that involves short-term culture of T lymphocytes and measurement of sister chromatid exchange ( SCE ) and chromosomal aberration frequency as genotoxic end-points .
	manualset3
101543	4	400373	5	NULL	NULL	NULL	NULL	genotoxicity	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In order to study individual differences in response to the genotoxicity of diepoxybutane , we devised a human lymphocyte culture system that involves short-term culture of T lymphocytes and measurement of sister chromatid exchange ( SCE ) and chromosomal aberration frequency as genotoxic end-points .
	manualset3
101544	5	400373	5	NULL	NULL	0	NULL	diepoxybutane	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to study individual differences in response to the genotoxicity of diepoxybutane , we devised a human lymphocyte culture system that involves short-term culture of T lymphocytes and measurement of sister chromatid exchange ( SCE ) and chromosomal aberration frequency as genotoxic end-points .
	manualset3
101545	6	400373	5	NULL	NULL	0	NULL	human lymphocyte culture system	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to study individual differences in response to the genotoxicity of diepoxybutane , we devised a human lymphocyte culture system that involves short-term culture of T lymphocytes and measurement of sister chromatid exchange ( SCE ) and chromosomal aberration frequency as genotoxic end-points .
	manualset3
101546	7	400373	5	NULL	NULL	0	NULL	short-term culture	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to study individual differences in response to the genotoxicity of diepoxybutane , we devised a human lymphocyte culture system that involves short-term culture of T lymphocytes and measurement of sister chromatid exchange ( SCE ) and chromosomal aberration frequency as genotoxic end-points .
	manualset3
101547	8	400373	5	NULL	NULL	0	NULL	T lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to study individual differences in response to the genotoxicity of diepoxybutane , we devised a human lymphocyte culture system that involves short-term culture of T lymphocytes and measurement of sister chromatid exchange ( SCE ) and chromosomal aberration frequency as genotoxic end-points .
	manualset3
101548	9	400373	5	NULL	NULL	0	NULL	measurement 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to study individual differences in response to the genotoxicity of diepoxybutane , we devised a human lymphocyte culture system that involves short-term culture of T lymphocytes and measurement of sister chromatid exchange ( SCE ) and chromosomal aberration frequency as genotoxic end-points .
	manualset3
101549	10	400373	5	NULL	NULL	0	NULL	sister chromatid exchange ( SCE ) and chromosomal aberration frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to study individual differences in response to the genotoxicity of diepoxybutane , we devised a human lymphocyte culture system that involves short-term culture of T lymphocytes and measurement of sister chromatid exchange ( SCE ) and chromosomal aberration frequency as genotoxic end-points .
	manualset3
101550	11	400373	5	NULL	NULL	0	NULL	 genotoxic end-points	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to study individual differences in response to the genotoxicity of diepoxybutane , we devised a human lymphocyte culture system that involves short-term culture of T lymphocytes and measurement of sister chromatid exchange ( SCE ) and chromosomal aberration frequency as genotoxic end-points .
	manualset3
101551	1	400374	5	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to study the distribution of bacteria as free floating in liquid and adherent to suspended particles , enumeration of the bacteria in the filterate and the sediment was also carried out .
	manualset3
101552	2	400374	5	NULL	NULL	0	NULL	distribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to study the distribution of bacteria as free floating in liquid and adherent to suspended particles , enumeration of the bacteria in the filterate and the sediment was also carried out .
	manualset3
101553	3	400374	5	NULL	NULL	0	NULL	bacteria 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to study the distribution of bacteria as free floating in liquid and adherent to suspended particles , enumeration of the bacteria in the filterate and the sediment was also carried out .
	manualset3
101554	4	400374	5	NULL	NULL	0	NULL	liquid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to study the distribution of bacteria as free floating in liquid and adherent to suspended particles , enumeration of the bacteria in the filterate and the sediment was also carried out .
	manualset3
101555	5	400374	5	NULL	NULL	0	NULL	suspended particles	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to study the distribution of bacteria as free floating in liquid and adherent to suspended particles , enumeration of the bacteria in the filterate and the sediment was also carried out .
	manualset3
101556	6	400374	5	NULL	NULL	0	NULL	enumeration 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to study the distribution of bacteria as free floating in liquid and adherent to suspended particles , enumeration of the bacteria in the filterate and the sediment was also carried out .
	manualset3
101557	7	400374	5	NULL	NULL	0	NULL	bacteria 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to study the distribution of bacteria as free floating in liquid and adherent to suspended particles , enumeration of the bacteria in the filterate and the sediment was also carried out .
	manualset3
101558	8	400374	5	NULL	NULL	0	NULL	filterate 	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to study the distribution of bacteria as free floating in liquid and adherent to suspended particles , enumeration of the bacteria in the filterate and the sediment was also carried out .
	manualset3
101559	9	400374	5	NULL	NULL	0	NULL	sediment 	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to study the distribution of bacteria as free floating in liquid and adherent to suspended particles , enumeration of the bacteria in the filterate and the sediment was also carried out .
	manualset3
101560	1	400375	5	NULL	NULL	0	NULL	 studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to support studies of short mackerel population genetic structure in the Gulf of Thailand and phylogenetic relationships , the mitochondrial genome of the short mackerel , Rastrelliger brachysoma , has recently been determined by a partial cloning technique , long PCR with three pairs of newly designed primers and primer walking sequencing .
	manualset3
101561	2	400375	5	NULL	NULL	0	NULL	short mackerel population genetic structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to support studies of short mackerel population genetic structure in the Gulf of Thailand and phylogenetic relationships , the mitochondrial genome of the short mackerel , Rastrelliger brachysoma , has recently been determined by a partial cloning technique , long PCR with three pairs of newly designed primers and primer walking sequencing .
	manualset3
101562	3	400375	5	NULL	NULL	0	NULL	Gulf of Thailand	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to support studies of short mackerel population genetic structure in the Gulf of Thailand and phylogenetic relationships , the mitochondrial genome of the short mackerel , Rastrelliger brachysoma , has recently been determined by a partial cloning technique , long PCR with three pairs of newly designed primers and primer walking sequencing .
	manualset3
101563	4	400375	5	NULL	NULL	0	NULL	phylogenetic relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to support studies of short mackerel population genetic structure in the Gulf of Thailand and phylogenetic relationships , the mitochondrial genome of the short mackerel , Rastrelliger brachysoma , has recently been determined by a partial cloning technique , long PCR with three pairs of newly designed primers and primer walking sequencing .
	manualset3
101564	5	400375	5	NULL	NULL	0	NULL	mitochondrial genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to support studies of short mackerel population genetic structure in the Gulf of Thailand and phylogenetic relationships , the mitochondrial genome of the short mackerel , Rastrelliger brachysoma , has recently been determined by a partial cloning technique , long PCR with three pairs of newly designed primers and primer walking sequencing .
	manualset3
101565	6	400375	5	NULL	NULL	0	NULL	short mackerel , Rastrelliger brachysoma	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to support studies of short mackerel population genetic structure in the Gulf of Thailand and phylogenetic relationships , the mitochondrial genome of the short mackerel , Rastrelliger brachysoma , has recently been determined by a partial cloning technique , long PCR with three pairs of newly designed primers and primer walking sequencing .
	manualset3
101566	7	400375	5	NULL	NULL	0	NULL	partial cloning technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to support studies of short mackerel population genetic structure in the Gulf of Thailand and phylogenetic relationships , the mitochondrial genome of the short mackerel , Rastrelliger brachysoma , has recently been determined by a partial cloning technique , long PCR with three pairs of newly designed primers and primer walking sequencing .
	manualset3
101567	8	400375	5	NULL	NULL	0	NULL	long PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to support studies of short mackerel population genetic structure in the Gulf of Thailand and phylogenetic relationships , the mitochondrial genome of the short mackerel , Rastrelliger brachysoma , has recently been determined by a partial cloning technique , long PCR with three pairs of newly designed primers and primer walking sequencing .
	manualset3
101568	9	400375	5	NULL	NULL	0	NULL	three pairs	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to support studies of short mackerel population genetic structure in the Gulf of Thailand and phylogenetic relationships , the mitochondrial genome of the short mackerel , Rastrelliger brachysoma , has recently been determined by a partial cloning technique , long PCR with three pairs of newly designed primers and primer walking sequencing .
	manualset3
101569	10	400375	5	NULL	NULL	0	NULL	newly designed primers	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to support studies of short mackerel population genetic structure in the Gulf of Thailand and phylogenetic relationships , the mitochondrial genome of the short mackerel , Rastrelliger brachysoma , has recently been determined by a partial cloning technique , long PCR with three pairs of newly designed primers and primer walking sequencing .
	manualset3
101570	11	400375	5	NULL	NULL	0	NULL	primer walking sequencing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to support studies of short mackerel population genetic structure in the Gulf of Thailand and phylogenetic relationships , the mitochondrial genome of the short mackerel , Rastrelliger brachysoma , has recently been determined by a partial cloning technique , long PCR with three pairs of newly designed primers and primer walking sequencing .
	manualset3
101571	1	400376	5	NULL	NULL	0	NULL	1994 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	, 366 : 704 , 1994 ; A. Kamb et al. , Science ( Washington DC ) , 264 : 436 , 1994 ; T. Nobori et al. , Nature ( Lond . )
	manualset3
101572	2	400376	5	NULL	NULL	NULL	NULL	A. Kamb et al. , Science ( Washington DC ) , 264 : 436 , 1994	Citation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	, 366 : 704 , 1994 ; A. Kamb et al. , Science ( Washington DC ) , 264 : 436 , 1994 ; T. Nobori et al. , Nature ( Lond . )
	manualset3
101573	3	400376	5	NULL	NULL	0	NULL	T. Nobori et al. , Nature ( Lond . ) 	Citation												NULL		0	NULL	NULL	NULL	NULL	NULL	, 366 : 704 , 1994 ; A. Kamb et al. , Science ( Washington DC ) , 264 : 436 , 1994 ; T. Nobori et al. , Nature ( Lond . )
	manualset3
101575	2	400377	5	NULL	NULL	0	NULL	association 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to understand the association of mitochondrial disorders with oxidative stress in obsessive compulsive disorder , we examined genetic variants of manganese superoxide dismutase and uncouple-2 antioxidant genes and malondialdehyde and glutathione , markers of oxidative stress .
	manualset3
101576	3	400377	5	NULL	NULL	0	NULL	mitochondrial disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to understand the association of mitochondrial disorders with oxidative stress in obsessive compulsive disorder , we examined genetic variants of manganese superoxide dismutase and uncouple-2 antioxidant genes and malondialdehyde and glutathione , markers of oxidative stress .
	manualset3
101577	4	400377	5	NULL	NULL	0	NULL	oxidative stress	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to understand the association of mitochondrial disorders with oxidative stress in obsessive compulsive disorder , we examined genetic variants of manganese superoxide dismutase and uncouple-2 antioxidant genes and malondialdehyde and glutathione , markers of oxidative stress .
	manualset3
101578	5	400377	5	NULL	NULL	0	NULL	obsessive compulsive disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to understand the association of mitochondrial disorders with oxidative stress in obsessive compulsive disorder , we examined genetic variants of manganese superoxide dismutase and uncouple-2 antioxidant genes and malondialdehyde and glutathione , markers of oxidative stress .
	manualset3
101579	6	400377	5	NULL	NULL	0	NULL	genetic variants	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to understand the association of mitochondrial disorders with oxidative stress in obsessive compulsive disorder , we examined genetic variants of manganese superoxide dismutase and uncouple-2 antioxidant genes and malondialdehyde and glutathione , markers of oxidative stress .
	manualset3
101580	7	400377	5	NULL	NULL	0	NULL	manganese superoxide dismutase	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to understand the association of mitochondrial disorders with oxidative stress in obsessive compulsive disorder , we examined genetic variants of manganese superoxide dismutase and uncouple-2 antioxidant genes and malondialdehyde and glutathione , markers of oxidative stress .
	manualset3
101581	8	400377	5	NULL	NULL	0	NULL	uncouple-2 antioxidant genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to understand the association of mitochondrial disorders with oxidative stress in obsessive compulsive disorder , we examined genetic variants of manganese superoxide dismutase and uncouple-2 antioxidant genes and malondialdehyde and glutathione , markers of oxidative stress .
	manualset3
101582	9	400377	5	NULL	NULL	0	NULL	malondialdehyde	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to understand the association of mitochondrial disorders with oxidative stress in obsessive compulsive disorder , we examined genetic variants of manganese superoxide dismutase and uncouple-2 antioxidant genes and malondialdehyde and glutathione , markers of oxidative stress .
	manualset3
101583	10	400377	5	NULL	NULL	0	NULL	glutathione 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to understand the association of mitochondrial disorders with oxidative stress in obsessive compulsive disorder , we examined genetic variants of manganese superoxide dismutase and uncouple-2 antioxidant genes and malondialdehyde and glutathione , markers of oxidative stress .
	manualset3
101584	11	400377	5	NULL	NULL	0	NULL	markers of oxidative stress	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to understand the association of mitochondrial disorders with oxidative stress in obsessive compulsive disorder , we examined genetic variants of manganese superoxide dismutase and uncouple-2 antioxidant genes and malondialdehyde and glutathione , markers of oxidative stress .
	manualset3
101585	1	400378	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to understand the effect of hematopoietic stem cell mobilization agents , G-CSF and GM-CSF , on the expression of TNF-alpha mRAN and CD69 and secretion of IgG in SLE patients ' peripheral blood mononuclear cells ( PBMNC ) , expression of TNF-alpha mRNA and CD69 was measured by RT-PCR and flow cytometry , respectively , and IgG secretion by ELISA .
	manualset3
101586	2	400378	5	NULL	NULL	0	NULL	hematopoietic stem cell mobilization agents	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to understand the effect of hematopoietic stem cell mobilization agents , G-CSF and GM-CSF , on the expression of TNF-alpha mRAN and CD69 and secretion of IgG in SLE patients ' peripheral blood mononuclear cells ( PBMNC ) , expression of TNF-alpha mRNA and CD69 was measured by RT-PCR and flow cytometry , respectively , and IgG secretion by ELISA .
	manualset3
101587	3	400378	5	NULL	NULL	0	NULL	G-CSF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to understand the effect of hematopoietic stem cell mobilization agents , G-CSF and GM-CSF , on the expression of TNF-alpha mRAN and CD69 and secretion of IgG in SLE patients ' peripheral blood mononuclear cells ( PBMNC ) , expression of TNF-alpha mRNA and CD69 was measured by RT-PCR and flow cytometry , respectively , and IgG secretion by ELISA .
	manualset3
101588	4	400378	5	NULL	NULL	0	NULL	GM-CSF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to understand the effect of hematopoietic stem cell mobilization agents , G-CSF and GM-CSF , on the expression of TNF-alpha mRAN and CD69 and secretion of IgG in SLE patients ' peripheral blood mononuclear cells ( PBMNC ) , expression of TNF-alpha mRNA and CD69 was measured by RT-PCR and flow cytometry , respectively , and IgG secretion by ELISA .
	manualset3
101589	5	400378	5	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to understand the effect of hematopoietic stem cell mobilization agents , G-CSF and GM-CSF , on the expression of TNF-alpha mRAN and CD69 and secretion of IgG in SLE patients ' peripheral blood mononuclear cells ( PBMNC ) , expression of TNF-alpha mRNA and CD69 was measured by RT-PCR and flow cytometry , respectively , and IgG secretion by ELISA .
	manualset3
101590	6	400378	5	NULL	NULL	0	NULL	TNF-alpha mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to understand the effect of hematopoietic stem cell mobilization agents , G-CSF and GM-CSF , on the expression of TNF-alpha mRAN and CD69 and secretion of IgG in SLE patients ' peripheral blood mononuclear cells ( PBMNC ) , expression of TNF-alpha mRNA and CD69 was measured by RT-PCR and flow cytometry , respectively , and IgG secretion by ELISA .
	manualset3
101591	7	400378	5	NULL	NULL	0	NULL	CD69	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to understand the effect of hematopoietic stem cell mobilization agents , G-CSF and GM-CSF , on the expression of TNF-alpha mRAN and CD69 and secretion of IgG in SLE patients ' peripheral blood mononuclear cells ( PBMNC ) , expression of TNF-alpha mRNA and CD69 was measured by RT-PCR and flow cytometry , respectively , and IgG secretion by ELISA .
	manualset3
101592	8	400378	5	NULL	NULL	NULL	NULL	secretion 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In order to understand the effect of hematopoietic stem cell mobilization agents , G-CSF and GM-CSF , on the expression of TNF-alpha mRAN and CD69 and secretion of IgG in SLE patients ' peripheral blood mononuclear cells ( PBMNC ) , expression of TNF-alpha mRNA and CD69 was measured by RT-PCR and flow cytometry , respectively , and IgG secretion by ELISA .
	manualset3
101593	9	400378	5	NULL	NULL	0	NULL	IgG	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to understand the effect of hematopoietic stem cell mobilization agents , G-CSF and GM-CSF , on the expression of TNF-alpha mRAN and CD69 and secretion of IgG in SLE patients ' peripheral blood mononuclear cells ( PBMNC ) , expression of TNF-alpha mRNA and CD69 was measured by RT-PCR and flow cytometry , respectively , and IgG secretion by ELISA .
	manualset3
101594	10	400378	5	NULL	NULL	0	NULL	SLE patients ' peripheral blood mononuclear cells ( PBMNC )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to understand the effect of hematopoietic stem cell mobilization agents , G-CSF and GM-CSF , on the expression of TNF-alpha mRAN and CD69 and secretion of IgG in SLE patients ' peripheral blood mononuclear cells ( PBMNC ) , expression of TNF-alpha mRNA and CD69 was measured by RT-PCR and flow cytometry , respectively , and IgG secretion by ELISA .
	manualset3
101595	11	400378	5	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to understand the effect of hematopoietic stem cell mobilization agents , G-CSF and GM-CSF , on the expression of TNF-alpha mRAN and CD69 and secretion of IgG in SLE patients ' peripheral blood mononuclear cells ( PBMNC ) , expression of TNF-alpha mRNA and CD69 was measured by RT-PCR and flow cytometry , respectively , and IgG secretion by ELISA .
	manualset3
101596	12	400378	5	NULL	NULL	0	NULL	TNF-alpha mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to understand the effect of hematopoietic stem cell mobilization agents , G-CSF and GM-CSF , on the expression of TNF-alpha mRAN and CD69 and secretion of IgG in SLE patients ' peripheral blood mononuclear cells ( PBMNC ) , expression of TNF-alpha mRNA and CD69 was measured by RT-PCR and flow cytometry , respectively , and IgG secretion by ELISA .
	manualset3
101597	13	400378	5	NULL	NULL	0	NULL	CD69	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to understand the effect of hematopoietic stem cell mobilization agents , G-CSF and GM-CSF , on the expression of TNF-alpha mRAN and CD69 and secretion of IgG in SLE patients ' peripheral blood mononuclear cells ( PBMNC ) , expression of TNF-alpha mRNA and CD69 was measured by RT-PCR and flow cytometry , respectively , and IgG secretion by ELISA .
	manualset3
101598	14	400378	5	NULL	NULL	0	NULL	RT-PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to understand the effect of hematopoietic stem cell mobilization agents , G-CSF and GM-CSF , on the expression of TNF-alpha mRAN and CD69 and secretion of IgG in SLE patients ' peripheral blood mononuclear cells ( PBMNC ) , expression of TNF-alpha mRNA and CD69 was measured by RT-PCR and flow cytometry , respectively , and IgG secretion by ELISA .
	manualset3
101599	15	400378	5	NULL	NULL	0	NULL	flow cytometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to understand the effect of hematopoietic stem cell mobilization agents , G-CSF and GM-CSF , on the expression of TNF-alpha mRAN and CD69 and secretion of IgG in SLE patients ' peripheral blood mononuclear cells ( PBMNC ) , expression of TNF-alpha mRNA and CD69 was measured by RT-PCR and flow cytometry , respectively , and IgG secretion by ELISA .
	manualset3
101600	16	400378	5	NULL	NULL	0	NULL	IgG secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to understand the effect of hematopoietic stem cell mobilization agents , G-CSF and GM-CSF , on the expression of TNF-alpha mRAN and CD69 and secretion of IgG in SLE patients ' peripheral blood mononuclear cells ( PBMNC ) , expression of TNF-alpha mRNA and CD69 was measured by RT-PCR and flow cytometry , respectively , and IgG secretion by ELISA .
	manualset3
101601	17	400378	5	NULL	NULL	0	NULL	ELISA 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to understand the effect of hematopoietic stem cell mobilization agents , G-CSF and GM-CSF , on the expression of TNF-alpha mRAN and CD69 and secretion of IgG in SLE patients ' peripheral blood mononuclear cells ( PBMNC ) , expression of TNF-alpha mRNA and CD69 was measured by RT-PCR and flow cytometry , respectively , and IgG secretion by ELISA .
	manualset3
101602	1	400379	5	NULL	NULL	0	NULL	verify	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to verify the established diagnosis , hemodynamic and BV changes during dialysis were studied .
	manualset3
101603	2	400379	5	NULL	NULL	0	NULL	established diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to verify the established diagnosis , hemodynamic and BV changes during dialysis were studied .
	manualset3
101604	3	400379	5	NULL	NULL	0	NULL	hemodynamic changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to verify the established diagnosis , hemodynamic and BV changes during dialysis were studied .
	manualset3
101605	4	400379	5	NULL	NULL	0	NULL	BV changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to verify the established diagnosis , hemodynamic and BV changes during dialysis were studied .
	manualset3
101606	5	400379	5	NULL	NULL	0	NULL	dialysis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to verify the established diagnosis , hemodynamic and BV changes during dialysis were studied .
	manualset3
101607	1	400380	5	NULL	NULL	0	NULL	verify	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to verify the new algorithm , it has been benchmarked against DOSXYZ and against measurements .
	manualset3
101608	2	400380	5	NULL	NULL	0	NULL	new algorithm	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to verify the new algorithm , it has been benchmarked against DOSXYZ and against measurements .
	manualset3
101609	3	400380	5	NULL	NULL	0	NULL	DOSXYZ 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to verify the new algorithm , it has been benchmarked against DOSXYZ and against measurements .
	manualset3
101610	4	400380	5	NULL	NULL	0	NULL	measurements	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to verify the new algorithm , it has been benchmarked against DOSXYZ and against measurements .
	manualset3
101611	1	400381	5	NULL	NULL	0	NULL	brain regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In other brain regions , including dentate gyrus and nucleus ambiguus , both receptor mRNAs were detected .
	manualset3
101612	2	400381	5	NULL	NULL	0	NULL	dentate gyrus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In other brain regions , including dentate gyrus and nucleus ambiguus , both receptor mRNAs were detected .
	manualset3
101613	3	400381	5	NULL	NULL	0	NULL	nucleus ambiguus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In other brain regions , including dentate gyrus and nucleus ambiguus , both receptor mRNAs were detected .
	manualset3
101614	4	400381	5	NULL	NULL	0	NULL	receptor mRNAs 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In other brain regions , including dentate gyrus and nucleus ambiguus , both receptor mRNAs were detected .
	manualset3
101615	1	400382	5	NULL	NULL	NULL	NULL	groups	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In other groups the thyroid lobes were incubated during exposure to CT and thyrotropin ( TSH ) , and to CGRP together with TSH .
	manualset3
101616	2	400382	5	NULL	NULL	0	NULL	thyroid lobes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In other groups the thyroid lobes were incubated during exposure to CT and thyrotropin ( TSH ) , and to CGRP together with TSH .
	manualset3
101617	3	400382	5	NULL	NULL	0	NULL	exposure 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In other groups the thyroid lobes were incubated during exposure to CT and thyrotropin ( TSH ) , and to CGRP together with TSH .
	manualset3
101618	4	400382	5	NULL	NULL	0	NULL	CT	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In other groups the thyroid lobes were incubated during exposure to CT and thyrotropin ( TSH ) , and to CGRP together with TSH .
	manualset3
101619	5	400382	5	NULL	NULL	0	NULL	thyrotropin ( TSH )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In other groups the thyroid lobes were incubated during exposure to CT and thyrotropin ( TSH ) , and to CGRP together with TSH .
	manualset3
101620	6	400382	5	NULL	NULL	0	NULL	CGRP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In other groups the thyroid lobes were incubated during exposure to CT and thyrotropin ( TSH ) , and to CGRP together with TSH .
	manualset3
101621	7	400382	5	NULL	NULL	0	NULL	TSH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In other groups the thyroid lobes were incubated during exposure to CT and thyrotropin ( TSH ) , and to CGRP together with TSH .
	manualset3
101622	1	400383	5	NULL	NULL	0	NULL	 increasingly networked world	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In our increasingly networked world , prizes are gaining a foothold in the race for innovation in science and technology .
	manualset3
101623	2	400383	5	NULL	NULL	0	NULL	prizes	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In our increasingly networked world , prizes are gaining a foothold in the race for innovation in science and technology .
	manualset3
101624	3	400383	5	NULL	NULL	0	NULL	foothold	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In our increasingly networked world , prizes are gaining a foothold in the race for innovation in science and technology .
	manualset3
101625	4	400383	5	NULL	NULL	0	NULL	race	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In our increasingly networked world , prizes are gaining a foothold in the race for innovation in science and technology .
	manualset3
101626	5	400383	5	NULL	NULL	0	NULL	innovation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In our increasingly networked world , prizes are gaining a foothold in the race for innovation in science and technology .
	manualset3
101627	6	400383	5	NULL	NULL	NULL	NULL	science and technology	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In our increasingly networked world , prizes are gaining a foothold in the race for innovation in science and technology .
	manualset3
101628	1	400384	5	NULL	NULL	0	NULL	laboratory 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In our laboratory we use a simple , fast and cost-effective approach to assess adequacy of FNAFNA materials and in this paper , we describe this procedure with giving some examples of interpretations of our results .
	manualset3
101629	2	400384	5	NULL	NULL	0	NULL	simple , fast and cost-effective approach	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In our laboratory we use a simple , fast and cost-effective approach to assess adequacy of FNAFNA materials and in this paper , we describe this procedure with giving some examples of interpretations of our results .
	manualset3
101631	4	400384	5	NULL	NULL	0	NULL	FNAFNA materials	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In our laboratory we use a simple , fast and cost-effective approach to assess adequacy of FNAFNA materials and in this paper , we describe this procedure with giving some examples of interpretations of our results .
	manualset3
101632	5	400384	5	NULL	NULL	0	NULL	paper 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In our laboratory we use a simple , fast and cost-effective approach to assess adequacy of FNAFNA materials and in this paper , we describe this procedure with giving some examples of interpretations of our results .
	manualset3
101633	6	400384	5	NULL	NULL	0	NULL	procedure 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In our laboratory we use a simple , fast and cost-effective approach to assess adequacy of FNAFNA materials and in this paper , we describe this procedure with giving some examples of interpretations of our results .
	manualset3
101634	7	400384	5	NULL	NULL	0	NULL	examples 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In our laboratory we use a simple , fast and cost-effective approach to assess adequacy of FNAFNA materials and in this paper , we describe this procedure with giving some examples of interpretations of our results .
	manualset3
101635	8	400384	5	NULL	NULL	0	NULL	interpretations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In our laboratory we use a simple , fast and cost-effective approach to assess adequacy of FNAFNA materials and in this paper , we describe this procedure with giving some examples of interpretations of our results .
	manualset3
101636	9	400384	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In our laboratory we use a simple , fast and cost-effective approach to assess adequacy of FNAFNA materials and in this paper , we describe this procedure with giving some examples of interpretations of our results .
	manualset3
101637	1	400385	5	NULL	NULL	0	NULL	previous studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In our previous studies , adenosine 3 ' , 5 ' - monophosphate ( cAMP ) was found to play an important role in this maturational process .
	manualset3
101638	2	400385	5	NULL	NULL	0	NULL	adenosine 3 ' , 5 ' - monophosphate ( cAMP )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In our previous studies , adenosine 3 ' , 5 ' - monophosphate ( cAMP ) was found to play an important role in this maturational process .
	manualset3
101639	3	400385	5	NULL	NULL	0	NULL	play an important role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In our previous studies , adenosine 3 ' , 5 ' - monophosphate ( cAMP ) was found to play an important role in this maturational process .
	manualset3
101640	4	400385	5	NULL	NULL	0	NULL	maturational process	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In our previous studies , adenosine 3 ' , 5 ' - monophosphate ( cAMP ) was found to play an important role in this maturational process .
	manualset3
101641	1	400386	5	NULL	NULL	0	NULL	53 cavernous angiomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In our series of 53 cavernous angiomas , all the 35 patients with preoperative seizures underwent surgery by means of lesionectomy alone .
	manualset3
101642	2	400386	5	NULL	NULL	0	NULL	35 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In our series of 53 cavernous angiomas , all the 35 patients with preoperative seizures underwent surgery by means of lesionectomy alone .
	manualset3
101643	3	400386	5	NULL	NULL	0	NULL	preoperative seizures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In our series of 53 cavernous angiomas , all the 35 patients with preoperative seizures underwent surgery by means of lesionectomy alone .
	manualset3
101644	4	400386	5	NULL	NULL	0	NULL	surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In our series of 53 cavernous angiomas , all the 35 patients with preoperative seizures underwent surgery by means of lesionectomy alone .
	manualset3
101645	5	400386	5	NULL	NULL	0	NULL	lesionectomy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In our series of 53 cavernous angiomas , all the 35 patients with preoperative seizures underwent surgery by means of lesionectomy alone .
	manualset3
101646	1	400387	5	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In our study , based on real-time single cell analysis , we investigated the molecular involvement of calpain in cisplatin-induced apoptosis in living human lung adenocarcinoma cells .
	manualset3
101647	2	400387	5	NULL	NULL	0	NULL	real-time single cell analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In our study , based on real-time single cell analysis , we investigated the molecular involvement of calpain in cisplatin-induced apoptosis in living human lung adenocarcinoma cells .
	manualset3
101648	3	400387	5	NULL	NULL	0	NULL	molecular involvement	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In our study , based on real-time single cell analysis , we investigated the molecular involvement of calpain in cisplatin-induced apoptosis in living human lung adenocarcinoma cells .
	manualset3
101649	4	400387	5	NULL	NULL	0	NULL	calpain 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In our study , based on real-time single cell analysis , we investigated the molecular involvement of calpain in cisplatin-induced apoptosis in living human lung adenocarcinoma cells .
	manualset3
101650	5	400387	5	NULL	NULL	0	NULL	cisplatin-induced apoptosis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In our study , based on real-time single cell analysis , we investigated the molecular involvement of calpain in cisplatin-induced apoptosis in living human lung adenocarcinoma cells .
	manualset3
101651	6	400387	5	NULL	NULL	0	NULL	living human lung adenocarcinoma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In our study , based on real-time single cell analysis , we investigated the molecular involvement of calpain in cisplatin-induced apoptosis in living human lung adenocarcinoma cells .
	manualset3
101652	1	400388	5	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In our study , we focused on the interesting non-acetylcholinesterase property of oximes , i.e. antinicotinic effect of reactivators .
	manualset3
101653	2	400388	5	NULL	NULL	0	NULL	non-acetylcholinesterase property	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In our study , we focused on the interesting non-acetylcholinesterase property of oximes , i.e. antinicotinic effect of reactivators .
	manualset3
101654	3	400388	5	NULL	NULL	0	NULL	oximes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In our study , we focused on the interesting non-acetylcholinesterase property of oximes , i.e. antinicotinic effect of reactivators .
	manualset3
101655	4	400388	5	NULL	NULL	0	NULL	antinicotinic effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In our study , we focused on the interesting non-acetylcholinesterase property of oximes , i.e. antinicotinic effect of reactivators .
	manualset3
101656	5	400388	5	NULL	NULL	0	NULL	reactivators 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In our study , we focused on the interesting non-acetylcholinesterase property of oximes , i.e. antinicotinic effect of reactivators .
	manualset3
101657	1	400389	5	NULL	NULL	0	NULL	outside-out patches	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In outside-out patches , lowering Ca2 + induces a single-channel current with a conductance of 36 pS .
	manualset3
101658	2	400389	5	NULL	NULL	0	NULL	 Ca2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In outside-out patches , lowering Ca2 + induces a single-channel current with a conductance of 36 pS .
	manualset3
101659	3	400389	5	NULL	NULL	0	NULL	single-channel current	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In outside-out patches , lowering Ca2 + induces a single-channel current with a conductance of 36 pS .
	manualset3
101660	4	400389	5	NULL	NULL	NULL	NULL	conductance 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In outside-out patches , lowering Ca2 + induces a single-channel current with a conductance of 36 pS .
	manualset3
101661	5	400389	5	NULL	NULL	0	NULL	36 pS	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In outside-out patches , lowering Ca2 + induces a single-channel current with a conductance of 36 pS .
	manualset3
101662	1	400390	5	NULL	NULL	0	NULL	paired t-tests	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In paired t-tests of the parameters under all conditions , there was a significant difference between test and retest .
	manualset3
101663	2	400390	5	NULL	NULL	0	NULL	parameters	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In paired t-tests of the parameters under all conditions , there was a significant difference between test and retest .
	manualset3
101664	3	400390	5	NULL	NULL	0	NULL	conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In paired t-tests of the parameters under all conditions , there was a significant difference between test and retest .
	manualset3
101665	4	400390	5	NULL	NULL	0	NULL	test 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In paired t-tests of the parameters under all conditions , there was a significant difference between test and retest .
	manualset3
101666	5	400390	5	NULL	NULL	0	NULL	retest 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In paired t-tests of the parameters under all conditions , there was a significant difference between test and retest .
	manualset3
101667	1	400391	5	NULL	NULL	0	NULL	infants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular that those infants with known clinical risk factors ( including cigarette smoke exposure , bed sharing and sleep position ) would have greater changes than those without clinical risks .
	manualset3
101668	2	400391	5	NULL	NULL	0	NULL	known clinical risk factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular that those infants with known clinical risk factors ( including cigarette smoke exposure , bed sharing and sleep position ) would have greater changes than those without clinical risks .
	manualset3
101669	3	400391	5	NULL	NULL	0	NULL	cigarette smoke exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular that those infants with known clinical risk factors ( including cigarette smoke exposure , bed sharing and sleep position ) would have greater changes than those without clinical risks .
	manualset3
101670	4	400391	5	NULL	NULL	0	NULL	bed sharing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular that those infants with known clinical risk factors ( including cigarette smoke exposure , bed sharing and sleep position ) would have greater changes than those without clinical risks .
	manualset3
101671	5	400391	5	NULL	NULL	0	NULL	sleep position	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular that those infants with known clinical risk factors ( including cigarette smoke exposure , bed sharing and sleep position ) would have greater changes than those without clinical risks .
	manualset3
101672	6	400391	5	NULL	NULL	0	NULL	changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular that those infants with known clinical risk factors ( including cigarette smoke exposure , bed sharing and sleep position ) would have greater changes than those without clinical risks .
	manualset3
101673	7	400391	5	NULL	NULL	0	NULL	clinical risks	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular that those infants with known clinical risk factors ( including cigarette smoke exposure , bed sharing and sleep position ) would have greater changes than those without clinical risks .
	manualset3
101674	1	400392	5	NULL	NULL	NULL	NULL	hatchery rainbow trout ( Oncorhynchus mykiss ) 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	, and hatchery rainbow trout ( Oncorhynchus mykiss ) , were tested with all three metals .
	manualset3
109521	2	400392	5	NULL	NULL	0	NULL	metals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	, and hatchery rainbow trout ( Oncorhynchus mykiss ) , were tested with all three metals .
	manualset3
101675	1	400393	5	NULL	NULL	0	NULL	 patient nos 1 and 2	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In patient nos 1 and 2 , histological examination showed that the arterial wall had been replaced by an abundant collagenic tissue .
	manualset3
101676	2	400393	5	NULL	NULL	0	NULL	histological examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In patient nos 1 and 2 , histological examination showed that the arterial wall had been replaced by an abundant collagenic tissue .
	manualset3
101677	3	400393	5	NULL	NULL	0	NULL	arterial wall	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In patient nos 1 and 2 , histological examination showed that the arterial wall had been replaced by an abundant collagenic tissue .
	manualset3
101678	4	400393	5	NULL	NULL	0	NULL	abundant collagenic tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In patient nos 1 and 2 , histological examination showed that the arterial wall had been replaced by an abundant collagenic tissue .
	manualset3
101679	1	400394	5	NULL	NULL	NULL	NULL	patients of group A	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In patients of group A revascularization prolonged significantly the load period during ergometry , as compared with medication ( from 7.2 + / - 2.2 min .
	manualset3
101680	2	400394	5	NULL	NULL	0	NULL	 revascularization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients of group A revascularization prolonged significantly the load period during ergometry , as compared with medication ( from 7.2 + / - 2.2 min .
	manualset3
101681	3	400394	5	NULL	NULL	0	NULL	load period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients of group A revascularization prolonged significantly the load period during ergometry , as compared with medication ( from 7.2 + / - 2.2 min .
	manualset3
101682	4	400394	5	NULL	NULL	0	NULL	ergometry 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients of group A revascularization prolonged significantly the load period during ergometry , as compared with medication ( from 7.2 + / - 2.2 min .
	manualset3
101683	5	400394	5	NULL	NULL	0	NULL	medication 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients of group A revascularization prolonged significantly the load period during ergometry , as compared with medication ( from 7.2 + / - 2.2 min .
	manualset3
101684	6	400394	5	NULL	NULL	NULL	NULL	from 7.2 + / - 2.2 min	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In patients of group A revascularization prolonged significantly the load period during ergometry , as compared with medication ( from 7.2 + / - 2.2 min .
	manualset3
101685	1	400395	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients on HD with cuprophan , apoptosis was higher than in control subjects and Non-D and CAPD patients .
	manualset3
101686	2	400395	5	NULL	NULL	0	NULL	HD	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients on HD with cuprophan , apoptosis was higher than in control subjects and Non-D and CAPD patients .
	manualset3
101687	3	400395	5	NULL	NULL	0	NULL	cuprophan 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients on HD with cuprophan , apoptosis was higher than in control subjects and Non-D and CAPD patients .
	manualset3
101688	4	400395	5	NULL	NULL	0	NULL	apoptosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients on HD with cuprophan , apoptosis was higher than in control subjects and Non-D and CAPD patients .
	manualset3
101689	5	400395	5	NULL	NULL	0	NULL	control subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients on HD with cuprophan , apoptosis was higher than in control subjects and Non-D and CAPD patients .
	manualset3
101690	6	400395	5	NULL	NULL	0	NULL	 Non-D patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients on HD with cuprophan , apoptosis was higher than in control subjects and Non-D and CAPD patients .
	manualset3
101691	7	400395	5	NULL	NULL	0	NULL	CAPD patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients on HD with cuprophan , apoptosis was higher than in control subjects and Non-D and CAPD patients .
	manualset3
101692	1	400396	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients presenting with urethral discharge in our rural setting , C. trachomatis was not found to be a major pathogen .
	manualset3
101693	2	400396	5	NULL	NULL	0	NULL	urethral discharge	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients presenting with urethral discharge in our rural setting , C. trachomatis was not found to be a major pathogen .
	manualset3
101694	3	400396	5	NULL	NULL	0	NULL	rural setting 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients presenting with urethral discharge in our rural setting , C. trachomatis was not found to be a major pathogen .
	manualset3
101695	4	400396	5	NULL	NULL	0	NULL	C. trachomatis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients presenting with urethral discharge in our rural setting , C. trachomatis was not found to be a major pathogen .
	manualset3
101696	5	400396	5	NULL	NULL	0	NULL	major pathogen	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients presenting with urethral discharge in our rural setting , C. trachomatis was not found to be a major pathogen .
	manualset3
101697	1	400397	5	NULL	NULL	0	NULL	patients 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients undergoing antibiotic treatment the faecal bacterial flora showed changes as a result of the use of the antibiotic .
	manualset3
101698	2	400397	5	NULL	NULL	0	NULL	antibiotic treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients undergoing antibiotic treatment the faecal bacterial flora showed changes as a result of the use of the antibiotic .
	manualset3
101699	3	400397	5	NULL	NULL	0	NULL	faecal bacterial flora	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients undergoing antibiotic treatment the faecal bacterial flora showed changes as a result of the use of the antibiotic .
	manualset3
101700	4	400397	5	NULL	NULL	0	NULL	changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients undergoing antibiotic treatment the faecal bacterial flora showed changes as a result of the use of the antibiotic .
	manualset3
101701	5	400397	5	NULL	NULL	0	NULL	result 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients undergoing antibiotic treatment the faecal bacterial flora showed changes as a result of the use of the antibiotic .
	manualset3
101702	6	400397	5	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients undergoing antibiotic treatment the faecal bacterial flora showed changes as a result of the use of the antibiotic .
	manualset3
101703	7	400397	5	NULL	NULL	0	NULL	antibiotic 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients undergoing antibiotic treatment the faecal bacterial flora showed changes as a result of the use of the antibiotic .
	manualset3
101704	1	400398	5	NULL	NULL	0	NULL	regionally advanced disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients who have regionally advanced disease , combination therapy consisting of concurrent chemotherapy and irradiation seems to have yielded an improvement in short-term and median survival .
	manualset3
101705	2	400398	5	NULL	NULL	0	NULL	combination therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients who have regionally advanced disease , combination therapy consisting of concurrent chemotherapy and irradiation seems to have yielded an improvement in short-term and median survival .
	manualset3
101706	3	400398	5	NULL	NULL	0	NULL	concurrent chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients who have regionally advanced disease , combination therapy consisting of concurrent chemotherapy and irradiation seems to have yielded an improvement in short-term and median survival .
	manualset3
101707	4	400398	5	NULL	NULL	0	NULL	irradiation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients who have regionally advanced disease , combination therapy consisting of concurrent chemotherapy and irradiation seems to have yielded an improvement in short-term and median survival .
	manualset3
101708	5	400398	5	NULL	NULL	0	NULL	improvement 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients who have regionally advanced disease , combination therapy consisting of concurrent chemotherapy and irradiation seems to have yielded an improvement in short-term and median survival .
	manualset3
101709	6	400398	5	NULL	NULL	0	NULL	short-term survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients who have regionally advanced disease , combination therapy consisting of concurrent chemotherapy and irradiation seems to have yielded an improvement in short-term and median survival .
	manualset3
101710	7	400398	5	NULL	NULL	0	NULL	median survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients who have regionally advanced disease , combination therapy consisting of concurrent chemotherapy and irradiation seems to have yielded an improvement in short-term and median survival .
	manualset3
109522	8	400398	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients who have regionally advanced disease , combination therapy consisting of concurrent chemotherapy and irradiation seems to have yielded an improvement in short-term and median survival .
	manualset3
101711	1	400399	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with DM2 , arrhythmias were associated with the duration of DM and HbA1c level .
	manualset3
101712	2	400399	5	NULL	NULL	0	NULL	DM2	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with DM2 , arrhythmias were associated with the duration of DM and HbA1c level .
	manualset3
101713	3	400399	5	NULL	NULL	0	NULL	arrhythmias 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with DM2 , arrhythmias were associated with the duration of DM and HbA1c level .
	manualset3
101714	4	400399	5	NULL	NULL	0	NULL	duration 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with DM2 , arrhythmias were associated with the duration of DM and HbA1c level .
	manualset3
101715	5	400399	5	NULL	NULL	0	NULL	DM level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with DM2 , arrhythmias were associated with the duration of DM and HbA1c level .
	manualset3
101716	6	400399	5	NULL	NULL	0	NULL	HbA1c level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with DM2 , arrhythmias were associated with the duration of DM and HbA1c level .
	manualset3
101717	1	400400	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with GFR & lt ; 25 ml/min x 1.73 m2 , all 99mTc-DTPA measurements were out of the 95 % confidence interval for the inulin measurement .
	manualset3
101718	2	400400	5	NULL	NULL	0	NULL	GFR 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with GFR & lt ; 25 ml/min x 1.73 m2 , all 99mTc-DTPA measurements were out of the 95 % confidence interval for the inulin measurement .
	manualset3
101719	3	400400	5	NULL	NULL	NULL	NULL	25 ml/min x 1.73 m2	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In patients with GFR & lt ; 25 ml/min x 1.73 m2 , all 99mTc-DTPA measurements were out of the 95 % confidence interval for the inulin measurement .
	manualset3
101720	4	400400	5	NULL	NULL	0	NULL	99mTc-DTPA measurements	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with GFR & lt ; 25 ml/min x 1.73 m2 , all 99mTc-DTPA measurements were out of the 95 % confidence interval for the inulin measurement .
	manualset3
101721	5	400400	5	NULL	NULL	0	NULL	95 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with GFR & lt ; 25 ml/min x 1.73 m2 , all 99mTc-DTPA measurements were out of the 95 % confidence interval for the inulin measurement .
	manualset3
101722	6	400400	5	NULL	NULL	0	NULL	confidence interval	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with GFR & lt ; 25 ml/min x 1.73 m2 , all 99mTc-DTPA measurements were out of the 95 % confidence interval for the inulin measurement .
	manualset3
101723	7	400400	5	NULL	NULL	0	NULL	inulin measurement	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with GFR & lt ; 25 ml/min x 1.73 m2 , all 99mTc-DTPA measurements were out of the 95 % confidence interval for the inulin measurement .
	manualset3
102259	1	400401	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with ILA , we observed an increased mean diffusivity ( MD ) and decreased levels of N-acetylaspartate ( NAA ) / creatine ( Cr ) in the anterior and posterior periventricular region and the thalamus , as well as decreased fractional anisotropy ( FA ) in the anterior and posterior periventricular regions .
	manualset3
102260	2	400401	5	NULL	NULL	0	NULL	ILA	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with ILA , we observed an increased mean diffusivity ( MD ) and decreased levels of N-acetylaspartate ( NAA ) / creatine ( Cr ) in the anterior and posterior periventricular region and the thalamus , as well as decreased fractional anisotropy ( FA ) in the anterior and posterior periventricular regions .
	manualset3
102261	3	400401	5	NULL	NULL	0	NULL	mean diffusivity ( MD )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with ILA , we observed an increased mean diffusivity ( MD ) and decreased levels of N-acetylaspartate ( NAA ) / creatine ( Cr ) in the anterior and posterior periventricular region and the thalamus , as well as decreased fractional anisotropy ( FA ) in the anterior and posterior periventricular regions .
	manualset3
102262	4	400401	5	NULL	NULL	0	NULL	decreased levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with ILA , we observed an increased mean diffusivity ( MD ) and decreased levels of N-acetylaspartate ( NAA ) / creatine ( Cr ) in the anterior and posterior periventricular region and the thalamus , as well as decreased fractional anisotropy ( FA ) in the anterior and posterior periventricular regions .
	manualset3
102263	5	400401	5	NULL	NULL	0	NULL	N-acetylaspartate ( NAA )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with ILA , we observed an increased mean diffusivity ( MD ) and decreased levels of N-acetylaspartate ( NAA ) / creatine ( Cr ) in the anterior and posterior periventricular region and the thalamus , as well as decreased fractional anisotropy ( FA ) in the anterior and posterior periventricular regions .
	manualset3
102264	6	400401	5	NULL	NULL	0	NULL	creatine ( Cr )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with ILA , we observed an increased mean diffusivity ( MD ) and decreased levels of N-acetylaspartate ( NAA ) / creatine ( Cr ) in the anterior and posterior periventricular region and the thalamus , as well as decreased fractional anisotropy ( FA ) in the anterior and posterior periventricular regions .
	manualset3
102265	7	400401	5	NULL	NULL	0	NULL	anterior and posterior periventricular region	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with ILA , we observed an increased mean diffusivity ( MD ) and decreased levels of N-acetylaspartate ( NAA ) / creatine ( Cr ) in the anterior and posterior periventricular region and the thalamus , as well as decreased fractional anisotropy ( FA ) in the anterior and posterior periventricular regions .
	manualset3
102266	8	400401	5	NULL	NULL	0	NULL	thalamus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with ILA , we observed an increased mean diffusivity ( MD ) and decreased levels of N-acetylaspartate ( NAA ) / creatine ( Cr ) in the anterior and posterior periventricular region and the thalamus , as well as decreased fractional anisotropy ( FA ) in the anterior and posterior periventricular regions .
	manualset3
102267	9	400401	5	NULL	NULL	0	NULL	decreased fractional anisotropy ( FA )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with ILA , we observed an increased mean diffusivity ( MD ) and decreased levels of N-acetylaspartate ( NAA ) / creatine ( Cr ) in the anterior and posterior periventricular region and the thalamus , as well as decreased fractional anisotropy ( FA ) in the anterior and posterior periventricular regions .
	manualset3
102268	10	400401	5	NULL	NULL	0	NULL	anterior and posterior periventricular regions	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with ILA , we observed an increased mean diffusivity ( MD ) and decreased levels of N-acetylaspartate ( NAA ) / creatine ( Cr ) in the anterior and posterior periventricular region and the thalamus , as well as decreased fractional anisotropy ( FA ) in the anterior and posterior periventricular regions .
	manualset3
102269	1	400402	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with LETM , a standardized diagnostic approach can result in a correct diagnosis and appropriate treatment .
	manualset3
102270	2	400402	5	NULL	NULL	0	NULL	LETM	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with LETM , a standardized diagnostic approach can result in a correct diagnosis and appropriate treatment .
	manualset3
102271	3	400402	5	NULL	NULL	0	NULL	standardized diagnostic approach	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with LETM , a standardized diagnostic approach can result in a correct diagnosis and appropriate treatment .
	manualset3
102272	4	400402	5	NULL	NULL	0	NULL	correct diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with LETM , a standardized diagnostic approach can result in a correct diagnosis and appropriate treatment .
	manualset3
102273	5	400402	5	NULL	NULL	0	NULL	appropriate treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with LETM , a standardized diagnostic approach can result in a correct diagnosis and appropriate treatment .
	manualset3
102274	1	400403	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with PAPLS and false positive serologic tests for Borrelia burgdorferi neurological involvement was significantly more common ( p = 0.012 , Fisher 's exact test ) than in patients with PAPLS without that finding .
	manualset3
102275	2	400403	5	NULL	NULL	0	NULL	PAPLS 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with PAPLS and false positive serologic tests for Borrelia burgdorferi neurological involvement was significantly more common ( p = 0.012 , Fisher 's exact test ) than in patients with PAPLS without that finding .
	manualset3
102276	3	400403	5	NULL	NULL	0	NULL	false positive serologic tests	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with PAPLS and false positive serologic tests for Borrelia burgdorferi neurological involvement was significantly more common ( p = 0.012 , Fisher 's exact test ) than in patients with PAPLS without that finding .
	manualset3
102277	4	400403	5	NULL	NULL	0	NULL	Borrelia burgdorferi neurological involvement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with PAPLS and false positive serologic tests for Borrelia burgdorferi neurological involvement was significantly more common ( p = 0.012 , Fisher 's exact test ) than in patients with PAPLS without that finding .
	manualset3
102278	4	400403	5	NULL	NULL	0	NULL	Borrelia burgdorferi neurological involvement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with PAPLS and false positive serologic tests for Borrelia burgdorferi neurological involvement was significantly more common ( p = 0.012 , Fisher 's exact test ) than in patients with PAPLS without that finding .
	manualset3
102279	5	400403	5	NULL	NULL	0	NULL	p = 0.012	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with PAPLS and false positive serologic tests for Borrelia burgdorferi neurological involvement was significantly more common ( p = 0.012 , Fisher 's exact test ) than in patients with PAPLS without that finding .
	manualset3
102280	6	400403	5	NULL	NULL	0	NULL	Fisher 's exact test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with PAPLS and false positive serologic tests for Borrelia burgdorferi neurological involvement was significantly more common ( p = 0.012 , Fisher 's exact test ) than in patients with PAPLS without that finding .
	manualset3
102281	7	400403	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with PAPLS and false positive serologic tests for Borrelia burgdorferi neurological involvement was significantly more common ( p = 0.012 , Fisher 's exact test ) than in patients with PAPLS without that finding .
	manualset3
102282	8	400403	5	NULL	NULL	0	NULL	PAPLS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with PAPLS and false positive serologic tests for Borrelia burgdorferi neurological involvement was significantly more common ( p = 0.012 , Fisher 's exact test ) than in patients with PAPLS without that finding .
	manualset3
109523	9	400403	5	NULL	NULL	0	NULL	finding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with PAPLS and false positive serologic tests for Borrelia burgdorferi neurological involvement was significantly more common ( p = 0.012 , Fisher 's exact test ) than in patients with PAPLS without that finding .
	manualset3
102283	1	400404	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with advanced gastric cancer , the response rate was reportedly over 40 % .
	manualset3
102284	2	400404	5	NULL	NULL	0	NULL	advanced gastric cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with advanced gastric cancer , the response rate was reportedly over 40 % .
	manualset3
102285	3	400404	5	NULL	NULL	0	NULL	response rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with advanced gastric cancer , the response rate was reportedly over 40 % .
	manualset3
102286	4	400404	5	NULL	NULL	0	NULL	40 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with advanced gastric cancer , the response rate was reportedly over 40 % .
	manualset3
102287	1	400405	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with advanced pancreatic NET , randomized , placebo-controlled studies have recently demonstrated that treatment with the tyrosine kinase inhibitor sunitinib or with mTOR inhibitor everolimus is associated with improved progression-free survival .
	manualset3
102288	2	400405	5	NULL	NULL	0	NULL	advanced pancreatic NET	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with advanced pancreatic NET , randomized , placebo-controlled studies have recently demonstrated that treatment with the tyrosine kinase inhibitor sunitinib or with mTOR inhibitor everolimus is associated with improved progression-free survival .
	manualset3
102290	3	400405	5	NULL	NULL	0	NULL	randomized , placebo-controlled studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with advanced pancreatic NET , randomized , placebo-controlled studies have recently demonstrated that treatment with the tyrosine kinase inhibitor sunitinib or with mTOR inhibitor everolimus is associated with improved progression-free survival .
	manualset3
102291	4	400405	5	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with advanced pancreatic NET , randomized , placebo-controlled studies have recently demonstrated that treatment with the tyrosine kinase inhibitor sunitinib or with mTOR inhibitor everolimus is associated with improved progression-free survival .
	manualset3
102292	5	400405	5	NULL	NULL	0	NULL	tyrosine kinase inhibitor sunitinib	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with advanced pancreatic NET , randomized , placebo-controlled studies have recently demonstrated that treatment with the tyrosine kinase inhibitor sunitinib or with mTOR inhibitor everolimus is associated with improved progression-free survival .
	manualset3
102293	6	400405	5	NULL	NULL	0	NULL	mTOR inhibitor everolimus	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with advanced pancreatic NET , randomized , placebo-controlled studies have recently demonstrated that treatment with the tyrosine kinase inhibitor sunitinib or with mTOR inhibitor everolimus is associated with improved progression-free survival .
	manualset3
102294	7	400405	5	NULL	NULL	0	NULL	improved progression-free survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with advanced pancreatic NET , randomized , placebo-controlled studies have recently demonstrated that treatment with the tyrosine kinase inhibitor sunitinib or with mTOR inhibitor everolimus is associated with improved progression-free survival .
	manualset3
102295	1	400406	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with an unperforated appendix no infections occurred after single-dose metronidazole prophylaxis as opposed to 8.2 % infections in untreated controls ( p less than 0.025 ) .
	manualset3
102296	2	400406	5	NULL	NULL	0	NULL	unperforated appendix	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with an unperforated appendix no infections occurred after single-dose metronidazole prophylaxis as opposed to 8.2 % infections in untreated controls ( p less than 0.025 ) .
	manualset3
102297	3	400406	5	NULL	NULL	0	NULL	infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with an unperforated appendix no infections occurred after single-dose metronidazole prophylaxis as opposed to 8.2 % infections in untreated controls ( p less than 0.025 ) .
	manualset3
102298	4	400406	5	NULL	NULL	0	NULL	single-dose metronidazole prophylaxis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with an unperforated appendix no infections occurred after single-dose metronidazole prophylaxis as opposed to 8.2 % infections in untreated controls ( p less than 0.025 ) .
	manualset3
102299	5	400406	5	NULL	NULL	0	NULL	8.2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with an unperforated appendix no infections occurred after single-dose metronidazole prophylaxis as opposed to 8.2 % infections in untreated controls ( p less than 0.025 ) .
	manualset3
102300	6	400406	5	NULL	NULL	0	NULL	infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with an unperforated appendix no infections occurred after single-dose metronidazole prophylaxis as opposed to 8.2 % infections in untreated controls ( p less than 0.025 ) .
	manualset3
102301	7	400406	5	NULL	NULL	0	NULL	untreated controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with an unperforated appendix no infections occurred after single-dose metronidazole prophylaxis as opposed to 8.2 % infections in untreated controls ( p less than 0.025 ) .
	manualset3
102302	8	400406	5	NULL	NULL	0	NULL	p less than 0.025	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with an unperforated appendix no infections occurred after single-dose metronidazole prophylaxis as opposed to 8.2 % infections in untreated controls ( p less than 0.025 ) .
	manualset3
102303	1	400407	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with cirrhosis of the liver protein content of ascites was low , LDH normal , and the ascites/serum ratio of glucose concentration was higher than 1 .
	manualset3
102304	2	400407	5	NULL	NULL	0	NULL	cirrhosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with cirrhosis of the liver protein content of ascites was low , LDH normal , and the ascites/serum ratio of glucose concentration was higher than 1 .
	manualset3
102305	3	400407	5	NULL	NULL	0	NULL	liver protein content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with cirrhosis of the liver protein content of ascites was low , LDH normal , and the ascites/serum ratio of glucose concentration was higher than 1 .
	manualset3
102306	4	400407	5	NULL	NULL	0	NULL	ascites	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with cirrhosis of the liver protein content of ascites was low , LDH normal , and the ascites/serum ratio of glucose concentration was higher than 1 .
	manualset3
102307	5	400407	5	NULL	NULL	0	NULL	LDH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with cirrhosis of the liver protein content of ascites was low , LDH normal , and the ascites/serum ratio of glucose concentration was higher than 1 .
	manualset3
102308	6	400407	5	NULL	NULL	0	NULL	ascites/serum ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with cirrhosis of the liver protein content of ascites was low , LDH normal , and the ascites/serum ratio of glucose concentration was higher than 1 .
	manualset3
102309	7	400407	5	NULL	NULL	0	NULL	glucose concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with cirrhosis of the liver protein content of ascites was low , LDH normal , and the ascites/serum ratio of glucose concentration was higher than 1 .
	manualset3
102310	8	400407	5	NULL	NULL	0	NULL	1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with cirrhosis of the liver protein content of ascites was low , LDH normal , and the ascites/serum ratio of glucose concentration was higher than 1 .
	manualset3
102311	1	400408	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with increased BMI , weight loss before transplantation reduces the risk of NODAT .
	manualset3
102312	2	400408	5	NULL	NULL	0	NULL	BMI	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with increased BMI , weight loss before transplantation reduces the risk of NODAT .
	manualset3
102313	3	400408	5	NULL	NULL	0	NULL	weight loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with increased BMI , weight loss before transplantation reduces the risk of NODAT .
	manualset3
102314	4	400408	5	NULL	NULL	0	NULL	transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with increased BMI , weight loss before transplantation reduces the risk of NODAT .
	manualset3
102315	5	400408	5	NULL	NULL	0	NULL	risk	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with increased BMI , weight loss before transplantation reduces the risk of NODAT .
	manualset3
102316	6	400408	5	NULL	NULL	0	NULL	NODAT	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with increased BMI , weight loss before transplantation reduces the risk of NODAT .
	manualset3
102317	1	400409	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with left bundle branch block ( LBBB ) and acute chest pain , the association between the clinical presentation and the diagnosis of myocardial infarction has not been investigated .
	manualset3
102318	2	400409	5	NULL	NULL	0	NULL	left bundle branch block ( LBBB )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with left bundle branch block ( LBBB ) and acute chest pain , the association between the clinical presentation and the diagnosis of myocardial infarction has not been investigated .
	manualset3
102319	3	400409	5	NULL	NULL	0	NULL	acute chest pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with left bundle branch block ( LBBB ) and acute chest pain , the association between the clinical presentation and the diagnosis of myocardial infarction has not been investigated .
	manualset3
102320	4	400409	5	NULL	NULL	0	NULL	association	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with left bundle branch block ( LBBB ) and acute chest pain , the association between the clinical presentation and the diagnosis of myocardial infarction has not been investigated .
	manualset3
102321	5	400409	5	NULL	NULL	NULL	NULL	clinical presentation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In patients with left bundle branch block ( LBBB ) and acute chest pain , the association between the clinical presentation and the diagnosis of myocardial infarction has not been investigated .
	manualset3
102322	6	400409	5	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with left bundle branch block ( LBBB ) and acute chest pain , the association between the clinical presentation and the diagnosis of myocardial infarction has not been investigated .
	manualset3
102323	7	400409	5	NULL	NULL	0	NULL	myocardial infarction	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with left bundle branch block ( LBBB ) and acute chest pain , the association between the clinical presentation and the diagnosis of myocardial infarction has not been investigated .
	manualset3
102324	1	400410	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients without seizures before therapy , seizures occurred during therapy in 5 of 82 patients ( 6 % ) receiving meropenem and in 1 of 86 patients ( 1 % ) receiving cefotaxime ( 95 % confidence interval : -0.7 % , 10.6 % ) .
	manualset3
102325	2	400410	5	NULL	NULL	0	NULL	seizures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients without seizures before therapy , seizures occurred during therapy in 5 of 82 patients ( 6 % ) receiving meropenem and in 1 of 86 patients ( 1 % ) receiving cefotaxime ( 95 % confidence interval : -0.7 % , 10.6 % ) .
	manualset3
102326	3	400410	5	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients without seizures before therapy , seizures occurred during therapy in 5 of 82 patients ( 6 % ) receiving meropenem and in 1 of 86 patients ( 1 % ) receiving cefotaxime ( 95 % confidence interval : -0.7 % , 10.6 % ) .
	manualset3
102327	4	400410	5	NULL	NULL	0	NULL	seizures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients without seizures before therapy , seizures occurred during therapy in 5 of 82 patients ( 6 % ) receiving meropenem and in 1 of 86 patients ( 1 % ) receiving cefotaxime ( 95 % confidence interval : -0.7 % , 10.6 % ) .
	manualset3
102328	5	400410	5	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients without seizures before therapy , seizures occurred during therapy in 5 of 82 patients ( 6 % ) receiving meropenem and in 1 of 86 patients ( 1 % ) receiving cefotaxime ( 95 % confidence interval : -0.7 % , 10.6 % ) .
	manualset3
102329	6	400410	5	NULL	NULL	0	NULL	5 of 82 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients without seizures before therapy , seizures occurred during therapy in 5 of 82 patients ( 6 % ) receiving meropenem and in 1 of 86 patients ( 1 % ) receiving cefotaxime ( 95 % confidence interval : -0.7 % , 10.6 % ) .
	manualset3
102330	7	400410	5	NULL	NULL	0	NULL	( 6 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients without seizures before therapy , seizures occurred during therapy in 5 of 82 patients ( 6 % ) receiving meropenem and in 1 of 86 patients ( 1 % ) receiving cefotaxime ( 95 % confidence interval : -0.7 % , 10.6 % ) .
	manualset3
102331	8	400410	5	NULL	NULL	0	NULL	meropenem	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients without seizures before therapy , seizures occurred during therapy in 5 of 82 patients ( 6 % ) receiving meropenem and in 1 of 86 patients ( 1 % ) receiving cefotaxime ( 95 % confidence interval : -0.7 % , 10.6 % ) .
	manualset3
102332	9	400410	5	NULL	NULL	0	NULL	1 of 86 patients	person												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients without seizures before therapy , seizures occurred during therapy in 5 of 82 patients ( 6 % ) receiving meropenem and in 1 of 86 patients ( 1 % ) receiving cefotaxime ( 95 % confidence interval : -0.7 % , 10.6 % ) .
	manualset3
102333	10	400410	5	NULL	NULL	0	NULL	( 1 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients without seizures before therapy , seizures occurred during therapy in 5 of 82 patients ( 6 % ) receiving meropenem and in 1 of 86 patients ( 1 % ) receiving cefotaxime ( 95 % confidence interval : -0.7 % , 10.6 % ) .
	manualset3
102334	11	400410	5	NULL	NULL	0	NULL	cefotaxime	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients without seizures before therapy , seizures occurred during therapy in 5 of 82 patients ( 6 % ) receiving meropenem and in 1 of 86 patients ( 1 % ) receiving cefotaxime ( 95 % confidence interval : -0.7 % , 10.6 % ) .
	manualset3
102335	12	400410	5	NULL	NULL	0	NULL	95 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients without seizures before therapy , seizures occurred during therapy in 5 of 82 patients ( 6 % ) receiving meropenem and in 1 of 86 patients ( 1 % ) receiving cefotaxime ( 95 % confidence interval : -0.7 % , 10.6 % ) .
	manualset3
102336	13	400410	5	NULL	NULL	0	NULL	confidence interval	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients without seizures before therapy , seizures occurred during therapy in 5 of 82 patients ( 6 % ) receiving meropenem and in 1 of 86 patients ( 1 % ) receiving cefotaxime ( 95 % confidence interval : -0.7 % , 10.6 % ) .
	manualset3
102337	14	400410	5	NULL	NULL	0	NULL	-0.7 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients without seizures before therapy , seizures occurred during therapy in 5 of 82 patients ( 6 % ) receiving meropenem and in 1 of 86 patients ( 1 % ) receiving cefotaxime ( 95 % confidence interval : -0.7 % , 10.6 % ) .
	manualset3
102338	15	400410	5	NULL	NULL	0	NULL	10.6 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients without seizures before therapy , seizures occurred during therapy in 5 of 82 patients ( 6 % ) receiving meropenem and in 1 of 86 patients ( 1 % ) receiving cefotaxime ( 95 % confidence interval : -0.7 % , 10.6 % ) .
	manualset3
102339	1	400411	5	NULL	NULL	0	NULL	persons	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In persons who chronically and continuously drink alcohol , there are demonstrable biochemical abnormalities similar to the effects of thyroid hormone on the liver .
	manualset3
102340	2	400411	5	NULL	NULL	NULL	NULL	alcohol	food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In persons who chronically and continuously drink alcohol , there are demonstrable biochemical abnormalities similar to the effects of thyroid hormone on the liver .
	manualset3
102341	3	400411	5	NULL	NULL	0	NULL	demonstrable biochemical abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In persons who chronically and continuously drink alcohol , there are demonstrable biochemical abnormalities similar to the effects of thyroid hormone on the liver .
	manualset3
102342	4	400411	5	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In persons who chronically and continuously drink alcohol , there are demonstrable biochemical abnormalities similar to the effects of thyroid hormone on the liver .
	manualset3
102343	5	400411	5	NULL	NULL	0	NULL	thyroid hormone	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In persons who chronically and continuously drink alcohol , there are demonstrable biochemical abnormalities similar to the effects of thyroid hormone on the liver .
	manualset3
102344	6	400411	5	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In persons who chronically and continuously drink alcohol , there are demonstrable biochemical abnormalities similar to the effects of thyroid hormone on the liver .
	manualset3
102345	1	400412	5	NULL	NULL	0	NULL	pharmacological studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In pharmacological studies , we observed that glycerol exerts a remarkable stabilizing effect on rhGM-CSF immunoreactivity .
	manualset3
102346	2	400412	5	NULL	NULL	0	NULL	glycerol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In pharmacological studies , we observed that glycerol exerts a remarkable stabilizing effect on rhGM-CSF immunoreactivity .
	manualset3
102347	3	400412	5	NULL	NULL	NULL	NULL	stabilizing effect	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In pharmacological studies , we observed that glycerol exerts a remarkable stabilizing effect on rhGM-CSF immunoreactivity .
	manualset3
102348	4	400412	5	NULL	NULL	0	NULL	rhGM-CSF immunoreactivity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In pharmacological studies , we observed that glycerol exerts a remarkable stabilizing effect on rhGM-CSF immunoreactivity .
	manualset3
102349	1	400413	5	NULL	NULL	0	NULL	pituitary-grafted male rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In pituitary-grafted male rats killed during spring , serum PRL levels were higher than controls at only a few time points throughout the 24 h cycle , whereas in rats killed during autumn , there were no significant differences in PRL levels between grafted and control rats .
	manualset3
102350	2	400413	5	NULL	NULL	0	NULL	spring	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In pituitary-grafted male rats killed during spring , serum PRL levels were higher than controls at only a few time points throughout the 24 h cycle , whereas in rats killed during autumn , there were no significant differences in PRL levels between grafted and control rats .
	manualset3
102351	3	400413	5	NULL	NULL	0	NULL	serum PRL levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In pituitary-grafted male rats killed during spring , serum PRL levels were higher than controls at only a few time points throughout the 24 h cycle , whereas in rats killed during autumn , there were no significant differences in PRL levels between grafted and control rats .
	manualset3
102352	4	400413	5	NULL	NULL	0	NULL	controls	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In pituitary-grafted male rats killed during spring , serum PRL levels were higher than controls at only a few time points throughout the 24 h cycle , whereas in rats killed during autumn , there were no significant differences in PRL levels between grafted and control rats .
	manualset3
102353	5	400413	5	NULL	NULL	0	NULL	time points	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	In pituitary-grafted male rats killed during spring , serum PRL levels were higher than controls at only a few time points throughout the 24 h cycle , whereas in rats killed during autumn , there were no significant differences in PRL levels between grafted and control rats .
	manualset3
102354	6	400413	5	NULL	NULL	0	NULL	24 h cycle	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In pituitary-grafted male rats killed during spring , serum PRL levels were higher than controls at only a few time points throughout the 24 h cycle , whereas in rats killed during autumn , there were no significant differences in PRL levels between grafted and control rats .
	manualset3
102355	7	400413	5	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In pituitary-grafted male rats killed during spring , serum PRL levels were higher than controls at only a few time points throughout the 24 h cycle , whereas in rats killed during autumn , there were no significant differences in PRL levels between grafted and control rats .
	manualset3
102356	8	400413	5	NULL	NULL	0	NULL	autumn	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In pituitary-grafted male rats killed during spring , serum PRL levels were higher than controls at only a few time points throughout the 24 h cycle , whereas in rats killed during autumn , there were no significant differences in PRL levels between grafted and control rats .
	manualset3
102357	9	400413	5	NULL	NULL	0	NULL	significant differences	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In pituitary-grafted male rats killed during spring , serum PRL levels were higher than controls at only a few time points throughout the 24 h cycle , whereas in rats killed during autumn , there were no significant differences in PRL levels between grafted and control rats .
	manualset3
102358	10	400413	5	NULL	NULL	0	NULL	PRL levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In pituitary-grafted male rats killed during spring , serum PRL levels were higher than controls at only a few time points throughout the 24 h cycle , whereas in rats killed during autumn , there were no significant differences in PRL levels between grafted and control rats .
	manualset3
102359	11	400413	5	NULL	NULL	0	NULL	grafted rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In pituitary-grafted male rats killed during spring , serum PRL levels were higher than controls at only a few time points throughout the 24 h cycle , whereas in rats killed during autumn , there were no significant differences in PRL levels between grafted and control rats .
	manualset3
102360	12	400413	5	NULL	NULL	0	NULL	control rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In pituitary-grafted male rats killed during spring , serum PRL levels were higher than controls at only a few time points throughout the 24 h cycle , whereas in rats killed during autumn , there were no significant differences in PRL levels between grafted and control rats .
	manualset3
102361	1	400414	5	NULL	NULL	0	NULL	places	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In places the epithelial cells appear edematous and vacuolated , and there is evidence of minute vesicle formation .
	manualset3
102362	2	400414	5	NULL	NULL	0	NULL	epithelial cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In places the epithelial cells appear edematous and vacuolated , and there is evidence of minute vesicle formation .
	manualset3
102363	3	400414	5	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In places the epithelial cells appear edematous and vacuolated , and there is evidence of minute vesicle formation .
	manualset3
102364	4	400414	5	NULL	NULL	0	NULL	minute vesicle formation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In places the epithelial cells appear edematous and vacuolated , and there is evidence of minute vesicle formation .
	manualset3
102365	1	400415	5	NULL	NULL	0	NULL	planning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In planning for pregnancy , one should discuss pregnancy outcomes and risks to both the mother and fetus .
	manualset3
102366	2	400415	5	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In planning for pregnancy , one should discuss pregnancy outcomes and risks to both the mother and fetus .
	manualset3
102367	3	400415	5	NULL	NULL	0	NULL	discuss	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In planning for pregnancy , one should discuss pregnancy outcomes and risks to both the mother and fetus .
	manualset3
102368	4	400415	5	NULL	NULL	0	NULL	pregnancy outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In planning for pregnancy , one should discuss pregnancy outcomes and risks to both the mother and fetus .
	manualset3
102369	5	400415	5	NULL	NULL	0	NULL	risks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In planning for pregnancy , one should discuss pregnancy outcomes and risks to both the mother and fetus .
	manualset3
102370	6	400415	5	NULL	NULL	0	NULL	mother	person												NULL		0	NULL	NULL	NULL	NULL	NULL	In planning for pregnancy , one should discuss pregnancy outcomes and risks to both the mother and fetus .
	manualset3
102371	7	400415	5	NULL	NULL	NULL	NULL	fetus	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In planning for pregnancy , one should discuss pregnancy outcomes and risks to both the mother and fetus .
	manualset3
102372	1	400416	5	NULL	NULL	0	NULL	preparation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In preparation for emerging plant virus epidemics , diagnostic manuals for economically important plant viruses that threaten local industries have been developed and validated under local conditions .
	manualset3
102373	2	400416	5	NULL	NULL	0	NULL	emerging plant virus epidemics	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In preparation for emerging plant virus epidemics , diagnostic manuals for economically important plant viruses that threaten local industries have been developed and validated under local conditions .
	manualset3
102374	3	400416	5	NULL	NULL	0	NULL	diagnostic manuals	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In preparation for emerging plant virus epidemics , diagnostic manuals for economically important plant viruses that threaten local industries have been developed and validated under local conditions .
	manualset3
102375	4	400416	5	NULL	NULL	0	NULL	economically important plant viruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In preparation for emerging plant virus epidemics , diagnostic manuals for economically important plant viruses that threaten local industries have been developed and validated under local conditions .
	manualset3
102376	5	400416	5	NULL	NULL	0	NULL	local industries	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In preparation for emerging plant virus epidemics , diagnostic manuals for economically important plant viruses that threaten local industries have been developed and validated under local conditions .
	manualset3
102377	6	400416	5	NULL	NULL	0	NULL	local conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In preparation for emerging plant virus epidemics , diagnostic manuals for economically important plant viruses that threaten local industries have been developed and validated under local conditions .
	manualset3
102378	1	400417	5	NULL	NULL	0	NULL	preparations	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In preparations treated with 0.3 microM ( - ) - Bay k 8644 , only the contractile responses to low concentrations of K + were inhibited by RP 49356 ( 0.1-1 .0 microM ) , cromakalim ( 0.1-1 .0 microM ) , nicorandil ( 1-10 microM ) , minoxidil sulphate ( 10 microM ) or HA 1004 ( 1 microM ) .
	manualset3
102379	2	400417	5	NULL	NULL	0	NULL	 0.3 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In preparations treated with 0.3 microM ( - ) - Bay k 8644 , only the contractile responses to low concentrations of K + were inhibited by RP 49356 ( 0.1-1 .0 microM ) , cromakalim ( 0.1-1 .0 microM ) , nicorandil ( 1-10 microM ) , minoxidil sulphate ( 10 microM ) or HA 1004 ( 1 microM ) .
	manualset3
102380	3	400417	5	NULL	NULL	0	NULL	Bay k 8644	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In preparations treated with 0.3 microM ( - ) - Bay k 8644 , only the contractile responses to low concentrations of K + were inhibited by RP 49356 ( 0.1-1 .0 microM ) , cromakalim ( 0.1-1 .0 microM ) , nicorandil ( 1-10 microM ) , minoxidil sulphate ( 10 microM ) or HA 1004 ( 1 microM ) .
	manualset3
102381	4	400417	5	NULL	NULL	0	NULL	contractile responses	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In preparations treated with 0.3 microM ( - ) - Bay k 8644 , only the contractile responses to low concentrations of K + were inhibited by RP 49356 ( 0.1-1 .0 microM ) , cromakalim ( 0.1-1 .0 microM ) , nicorandil ( 1-10 microM ) , minoxidil sulphate ( 10 microM ) or HA 1004 ( 1 microM ) .
	manualset3
102382	5	400417	5	NULL	NULL	0	NULL	low concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In preparations treated with 0.3 microM ( - ) - Bay k 8644 , only the contractile responses to low concentrations of K + were inhibited by RP 49356 ( 0.1-1 .0 microM ) , cromakalim ( 0.1-1 .0 microM ) , nicorandil ( 1-10 microM ) , minoxidil sulphate ( 10 microM ) or HA 1004 ( 1 microM ) .
	manualset3
102383	6	400417	5	NULL	NULL	0	NULL	K +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In preparations treated with 0.3 microM ( - ) - Bay k 8644 , only the contractile responses to low concentrations of K + were inhibited by RP 49356 ( 0.1-1 .0 microM ) , cromakalim ( 0.1-1 .0 microM ) , nicorandil ( 1-10 microM ) , minoxidil sulphate ( 10 microM ) or HA 1004 ( 1 microM ) .
	manualset3
102384	7	400417	5	NULL	NULL	0	NULL	RP 49356	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In preparations treated with 0.3 microM ( - ) - Bay k 8644 , only the contractile responses to low concentrations of K + were inhibited by RP 49356 ( 0.1-1 .0 microM ) , cromakalim ( 0.1-1 .0 microM ) , nicorandil ( 1-10 microM ) , minoxidil sulphate ( 10 microM ) or HA 1004 ( 1 microM ) .
	manualset3
102385	8	400417	5	NULL	NULL	0	NULL	0.1-1 .0 microM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In preparations treated with 0.3 microM ( - ) - Bay k 8644 , only the contractile responses to low concentrations of K + were inhibited by RP 49356 ( 0.1-1 .0 microM ) , cromakalim ( 0.1-1 .0 microM ) , nicorandil ( 1-10 microM ) , minoxidil sulphate ( 10 microM ) or HA 1004 ( 1 microM ) .
	manualset3
102386	9	400417	5	NULL	NULL	0	NULL	cromakalim	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In preparations treated with 0.3 microM ( - ) - Bay k 8644 , only the contractile responses to low concentrations of K + were inhibited by RP 49356 ( 0.1-1 .0 microM ) , cromakalim ( 0.1-1 .0 microM ) , nicorandil ( 1-10 microM ) , minoxidil sulphate ( 10 microM ) or HA 1004 ( 1 microM ) .
	manualset3
102387	10	400417	5	NULL	NULL	0	NULL	 0.1-1 .0 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In preparations treated with 0.3 microM ( - ) - Bay k 8644 , only the contractile responses to low concentrations of K + were inhibited by RP 49356 ( 0.1-1 .0 microM ) , cromakalim ( 0.1-1 .0 microM ) , nicorandil ( 1-10 microM ) , minoxidil sulphate ( 10 microM ) or HA 1004 ( 1 microM ) .
	manualset3
102388	11	400417	5	NULL	NULL	0	NULL	nicorandil	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In preparations treated with 0.3 microM ( - ) - Bay k 8644 , only the contractile responses to low concentrations of K + were inhibited by RP 49356 ( 0.1-1 .0 microM ) , cromakalim ( 0.1-1 .0 microM ) , nicorandil ( 1-10 microM ) , minoxidil sulphate ( 10 microM ) or HA 1004 ( 1 microM ) .
	manualset3
102389	12	400417	5	NULL	NULL	0	NULL	1-10 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In preparations treated with 0.3 microM ( - ) - Bay k 8644 , only the contractile responses to low concentrations of K + were inhibited by RP 49356 ( 0.1-1 .0 microM ) , cromakalim ( 0.1-1 .0 microM ) , nicorandil ( 1-10 microM ) , minoxidil sulphate ( 10 microM ) or HA 1004 ( 1 microM ) .
	manualset3
102390	13	400417	5	NULL	NULL	0	NULL	minoxidil sulphate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In preparations treated with 0.3 microM ( - ) - Bay k 8644 , only the contractile responses to low concentrations of K + were inhibited by RP 49356 ( 0.1-1 .0 microM ) , cromakalim ( 0.1-1 .0 microM ) , nicorandil ( 1-10 microM ) , minoxidil sulphate ( 10 microM ) or HA 1004 ( 1 microM ) .
	manualset3
102391	14	400417	5	NULL	NULL	0	NULL	10 microM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In preparations treated with 0.3 microM ( - ) - Bay k 8644 , only the contractile responses to low concentrations of K + were inhibited by RP 49356 ( 0.1-1 .0 microM ) , cromakalim ( 0.1-1 .0 microM ) , nicorandil ( 1-10 microM ) , minoxidil sulphate ( 10 microM ) or HA 1004 ( 1 microM ) .
	manualset3
102654	15	400417	5	NULL	NULL	0	NULL	HA 1004	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In preparations treated with 0.3 microM ( - ) - Bay k 8644 , only the contractile responses to low concentrations of K + were inhibited by RP 49356 ( 0.1-1 .0 microM ) , cromakalim ( 0.1-1 .0 microM ) , nicorandil ( 1-10 microM ) , minoxidil sulphate ( 10 microM ) or HA 1004 ( 1 microM ) .
	manualset3
102655	16	400417	5	NULL	NULL	0	NULL	1 microM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In preparations treated with 0.3 microM ( - ) - Bay k 8644 , only the contractile responses to low concentrations of K + were inhibited by RP 49356 ( 0.1-1 .0 microM ) , cromakalim ( 0.1-1 .0 microM ) , nicorandil ( 1-10 microM ) , minoxidil sulphate ( 10 microM ) or HA 1004 ( 1 microM ) .
	manualset3
102656	1	400418	5	NULL	NULL	0	NULL	publications 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous publications ( Diederen , 1972 , 1973 ) evidence was presented that light and darkness hardly influence the secretory activity of the subcommissural organ ( SCO ) in intact frogs , i.e. frogs in which all photo-receptive organs are present .
	manualset3
102657	2	400418	5	NULL	NULL	0	NULL	Diederen 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous publications ( Diederen , 1972 , 1973 ) evidence was presented that light and darkness hardly influence the secretory activity of the subcommissural organ ( SCO ) in intact frogs , i.e. frogs in which all photo-receptive organs are present .
	manualset3
102658	3	400418	5	NULL	NULL	0	NULL	1972	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous publications ( Diederen , 1972 , 1973 ) evidence was presented that light and darkness hardly influence the secretory activity of the subcommissural organ ( SCO ) in intact frogs , i.e. frogs in which all photo-receptive organs are present .
	manualset3
102659	4	400418	5	NULL	NULL	0	NULL	1973	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous publications ( Diederen , 1972 , 1973 ) evidence was presented that light and darkness hardly influence the secretory activity of the subcommissural organ ( SCO ) in intact frogs , i.e. frogs in which all photo-receptive organs are present .
	manualset3
102660	5	400418	5	NULL	NULL	0	NULL	evidence	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous publications ( Diederen , 1972 , 1973 ) evidence was presented that light and darkness hardly influence the secretory activity of the subcommissural organ ( SCO ) in intact frogs , i.e. frogs in which all photo-receptive organs are present .
	manualset3
102661	6	400418	5	NULL	NULL	0	NULL	light	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous publications ( Diederen , 1972 , 1973 ) evidence was presented that light and darkness hardly influence the secretory activity of the subcommissural organ ( SCO ) in intact frogs , i.e. frogs in which all photo-receptive organs are present .
	manualset3
102662	7	400418	5	NULL	NULL	0	NULL	darkness	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous publications ( Diederen , 1972 , 1973 ) evidence was presented that light and darkness hardly influence the secretory activity of the subcommissural organ ( SCO ) in intact frogs , i.e. frogs in which all photo-receptive organs are present .
	manualset3
102664	8	400418	5	NULL	NULL	0	NULL	secretory activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous publications ( Diederen , 1972 , 1973 ) evidence was presented that light and darkness hardly influence the secretory activity of the subcommissural organ ( SCO ) in intact frogs , i.e. frogs in which all photo-receptive organs are present .
	manualset3
102665	9	400418	5	NULL	NULL	0	NULL	subcommissural organ ( SCO )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous publications ( Diederen , 1972 , 1973 ) evidence was presented that light and darkness hardly influence the secretory activity of the subcommissural organ ( SCO ) in intact frogs , i.e. frogs in which all photo-receptive organs are present .
	manualset3
102667	10	400418	5	NULL	NULL	0	NULL	intact frogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous publications ( Diederen , 1972 , 1973 ) evidence was presented that light and darkness hardly influence the secretory activity of the subcommissural organ ( SCO ) in intact frogs , i.e. frogs in which all photo-receptive organs are present .
	manualset3
102668	11	400418	5	NULL	NULL	0	NULL	frogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous publications ( Diederen , 1972 , 1973 ) evidence was presented that light and darkness hardly influence the secretory activity of the subcommissural organ ( SCO ) in intact frogs , i.e. frogs in which all photo-receptive organs are present .
	manualset3
109524	12	400418	5	NULL	NULL	0	NULL	photo-receptive organs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous publications ( Diederen , 1972 , 1973 ) evidence was presented that light and darkness hardly influence the secretory activity of the subcommissural organ ( SCO ) in intact frogs , i.e. frogs in which all photo-receptive organs are present .
	manualset3
102669	1	400419	5	NULL	NULL	0	NULL	reports	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous reports an arthrotomy was used to accomplish this repair ; in this paper an arthroscopic technique is presented .
	manualset3
102673	2	400419	5	NULL	NULL	0	NULL	arthrotomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous reports an arthrotomy was used to accomplish this repair ; in this paper an arthroscopic technique is presented .
	manualset3
102674	3	400419	5	NULL	NULL	0	NULL	repair	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous reports an arthrotomy was used to accomplish this repair ; in this paper an arthroscopic technique is presented .
	manualset3
102675	4	400419	5	NULL	NULL	0	NULL	paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous reports an arthrotomy was used to accomplish this repair ; in this paper an arthroscopic technique is presented .
	manualset3
102677	5	400419	5	NULL	NULL	0	NULL	arthroscopic technique	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous reports an arthrotomy was used to accomplish this repair ; in this paper an arthroscopic technique is presented .
	manualset3
102681	1	400420	5	NULL	NULL	0	NULL	previous studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous studies , the read-out was performed by atomic force microscopy ( AFM ) , but in our work SXCM microradiographs were imaged by scanning ion microscopy ( SIM ) in a focused ion beam/scanning electron microscope ( FIB/SEM ) .
	manualset3
102682	2	400420	5	NULL	NULL	0	NULL	read-out	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous studies , the read-out was performed by atomic force microscopy ( AFM ) , but in our work SXCM microradiographs were imaged by scanning ion microscopy ( SIM ) in a focused ion beam/scanning electron microscope ( FIB/SEM ) .
	manualset3
102683	3	400420	5	NULL	NULL	0	NULL	atomic force microscopy ( AFM )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous studies , the read-out was performed by atomic force microscopy ( AFM ) , but in our work SXCM microradiographs were imaged by scanning ion microscopy ( SIM ) in a focused ion beam/scanning electron microscope ( FIB/SEM ) .
	manualset3
102684	4	400420	5	NULL	NULL	0	NULL	work	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous studies , the read-out was performed by atomic force microscopy ( AFM ) , but in our work SXCM microradiographs were imaged by scanning ion microscopy ( SIM ) in a focused ion beam/scanning electron microscope ( FIB/SEM ) .
	manualset3
102685	5	400420	5	NULL	NULL	0	NULL	SXCM microradiographs	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous studies , the read-out was performed by atomic force microscopy ( AFM ) , but in our work SXCM microradiographs were imaged by scanning ion microscopy ( SIM ) in a focused ion beam/scanning electron microscope ( FIB/SEM ) .
	manualset3
102686	6	400420	5	NULL	NULL	0	NULL	scanning ion microscopy ( SIM )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous studies , the read-out was performed by atomic force microscopy ( AFM ) , but in our work SXCM microradiographs were imaged by scanning ion microscopy ( SIM ) in a focused ion beam/scanning electron microscope ( FIB/SEM ) .
	manualset3
102687	7	400420	5	NULL	NULL	0	NULL	ion beam/scanning electron microscope ( FIB/SEM )	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous studies , the read-out was performed by atomic force microscopy ( AFM ) , but in our work SXCM microradiographs were imaged by scanning ion microscopy ( SIM ) in a focused ion beam/scanning electron microscope ( FIB/SEM ) .
	manualset3
102689	1	400421	5	NULL	NULL	0	NULL	previous studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous studies mice bearing an established transplanted syngeneic leukemia were cured by the adoptive transfer of immune lymphoid cells inoculated as an adjunct to chemotherapy , whereas nonimmune cells had no effect .
	manualset3
102691	2	400421	5	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous studies mice bearing an established transplanted syngeneic leukemia were cured by the adoptive transfer of immune lymphoid cells inoculated as an adjunct to chemotherapy , whereas nonimmune cells had no effect .
	manualset3
102693	3	400421	5	NULL	NULL	0	NULL	transplanted syngeneic leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous studies mice bearing an established transplanted syngeneic leukemia were cured by the adoptive transfer of immune lymphoid cells inoculated as an adjunct to chemotherapy , whereas nonimmune cells had no effect .
	manualset3
102694	4	400421	5	NULL	NULL	0	NULL	adoptive transfer	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous studies mice bearing an established transplanted syngeneic leukemia were cured by the adoptive transfer of immune lymphoid cells inoculated as an adjunct to chemotherapy , whereas nonimmune cells had no effect .
	manualset3
102696	5	400421	5	NULL	NULL	0	NULL	immune lymphoid cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous studies mice bearing an established transplanted syngeneic leukemia were cured by the adoptive transfer of immune lymphoid cells inoculated as an adjunct to chemotherapy , whereas nonimmune cells had no effect .
	manualset3
102700	6	400421	5	NULL	NULL	0	NULL	adjunct	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous studies mice bearing an established transplanted syngeneic leukemia were cured by the adoptive transfer of immune lymphoid cells inoculated as an adjunct to chemotherapy , whereas nonimmune cells had no effect .
	manualset3
102701	7	400421	5	NULL	NULL	0	NULL	chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous studies mice bearing an established transplanted syngeneic leukemia were cured by the adoptive transfer of immune lymphoid cells inoculated as an adjunct to chemotherapy , whereas nonimmune cells had no effect .
	manualset3
102702	8	400421	5	NULL	NULL	0	NULL	nonimmune cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous studies mice bearing an established transplanted syngeneic leukemia were cured by the adoptive transfer of immune lymphoid cells inoculated as an adjunct to chemotherapy , whereas nonimmune cells had no effect .
	manualset3
102703	9	400421	5	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous studies mice bearing an established transplanted syngeneic leukemia were cured by the adoptive transfer of immune lymphoid cells inoculated as an adjunct to chemotherapy , whereas nonimmune cells had no effect .
	manualset3
102706	1	400422	5	NULL	NULL	0	NULL	previous work 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous work on the mixed-mode loading of human cortical bone ( using an asymmetric bend test geometry ) , we found that the bone toughness was lower when loaded in far-field shear than in tension ( opposite to the trend in most brittle materials ) , although only for the transverse orientation .
	manualset3
102711	2	400422	5	NULL	NULL	0	NULL	mixed-mode loading	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous work on the mixed-mode loading of human cortical bone ( using an asymmetric bend test geometry ) , we found that the bone toughness was lower when loaded in far-field shear than in tension ( opposite to the trend in most brittle materials ) , although only for the transverse orientation .
	manualset3
102712	3	400422	5	NULL	NULL	0	NULL	human cortical bone	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous work on the mixed-mode loading of human cortical bone ( using an asymmetric bend test geometry ) , we found that the bone toughness was lower when loaded in far-field shear than in tension ( opposite to the trend in most brittle materials ) , although only for the transverse orientation .
	manualset3
102713	4	400422	5	NULL	NULL	0	NULL	asymmetric bend test geometry	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous work on the mixed-mode loading of human cortical bone ( using an asymmetric bend test geometry ) , we found that the bone toughness was lower when loaded in far-field shear than in tension ( opposite to the trend in most brittle materials ) , although only for the transverse orientation .
	manualset3
102714	5	400422	5	NULL	NULL	0	NULL	bone toughness	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous work on the mixed-mode loading of human cortical bone ( using an asymmetric bend test geometry ) , we found that the bone toughness was lower when loaded in far-field shear than in tension ( opposite to the trend in most brittle materials ) , although only for the transverse orientation .
	manualset3
102723	6	400422	5	NULL	NULL	0	NULL	far-field shear	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous work on the mixed-mode loading of human cortical bone ( using an asymmetric bend test geometry ) , we found that the bone toughness was lower when loaded in far-field shear than in tension ( opposite to the trend in most brittle materials ) , although only for the transverse orientation .
	manualset3
102725	7	400422	5	NULL	NULL	0	NULL	tension 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous work on the mixed-mode loading of human cortical bone ( using an asymmetric bend test geometry ) , we found that the bone toughness was lower when loaded in far-field shear than in tension ( opposite to the trend in most brittle materials ) , although only for the transverse orientation .
	manualset3
102726	8	400422	5	NULL	NULL	0	NULL	brittle materials	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous work on the mixed-mode loading of human cortical bone ( using an asymmetric bend test geometry ) , we found that the bone toughness was lower when loaded in far-field shear than in tension ( opposite to the trend in most brittle materials ) , although only for the transverse orientation .
	manualset3
102727	9	400422	5	NULL	NULL	0	NULL	transverse orientation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous work on the mixed-mode loading of human cortical bone ( using an asymmetric bend test geometry ) , we found that the bone toughness was lower when loaded in far-field shear than in tension ( opposite to the trend in most brittle materials ) , although only for the transverse orientation .
	manualset3
102728	1	400423	5	NULL	NULL	0	NULL	protoplasts 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In protoplasts coinoculated with BMV RNA1 and RNA2 , the nonamplifiable RNA3 derivatives bearing TMV 3 ' sequences gave rise to diverse new rearranged or recombined RNA species that were amplifiable .
	manualset3
102729	2	400423	5	NULL	NULL	0	NULL	BMV RNA1	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In protoplasts coinoculated with BMV RNA1 and RNA2 , the nonamplifiable RNA3 derivatives bearing TMV 3 ' sequences gave rise to diverse new rearranged or recombined RNA species that were amplifiable .
	manualset3
102730	3	400423	5	NULL	NULL	0	NULL	BMV RNA2	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In protoplasts coinoculated with BMV RNA1 and RNA2 , the nonamplifiable RNA3 derivatives bearing TMV 3 ' sequences gave rise to diverse new rearranged or recombined RNA species that were amplifiable .
	manualset3
102731	4	400423	5	NULL	NULL	0	NULL	nonamplifiable RNA3 derivatives bearing TMV 3 ' sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In protoplasts coinoculated with BMV RNA1 and RNA2 , the nonamplifiable RNA3 derivatives bearing TMV 3 ' sequences gave rise to diverse new rearranged or recombined RNA species that were amplifiable .
	manualset3
102732	5	400423	5	NULL	NULL	0	NULL	diverse new rearranged RNA species	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In protoplasts coinoculated with BMV RNA1 and RNA2 , the nonamplifiable RNA3 derivatives bearing TMV 3 ' sequences gave rise to diverse new rearranged or recombined RNA species that were amplifiable .
	manualset3
102733	1	400424	5	NULL	NULL	0	NULL	 pulse-chase experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In pulse-chase experiments , the pattern of loss of the incorporated fatty acid was similar to that of the protein itself , and therefore the loss of radioactivity probably reflects protein degradation rather than specific de-acylation of the protein .
	manualset3
102734	2	400424	5	NULL	NULL	0	NULL	pattern of loss	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In pulse-chase experiments , the pattern of loss of the incorporated fatty acid was similar to that of the protein itself , and therefore the loss of radioactivity probably reflects protein degradation rather than specific de-acylation of the protein .
	manualset3
102735	3	400424	5	NULL	NULL	0	NULL	incorporated fatty acid	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In pulse-chase experiments , the pattern of loss of the incorporated fatty acid was similar to that of the protein itself , and therefore the loss of radioactivity probably reflects protein degradation rather than specific de-acylation of the protein .
	manualset3
102736	4	400424	5	NULL	NULL	0	NULL	protein 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In pulse-chase experiments , the pattern of loss of the incorporated fatty acid was similar to that of the protein itself , and therefore the loss of radioactivity probably reflects protein degradation rather than specific de-acylation of the protein .
	manualset3
102737	5	400424	5	NULL	NULL	0	NULL	loss of radioactivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In pulse-chase experiments , the pattern of loss of the incorporated fatty acid was similar to that of the protein itself , and therefore the loss of radioactivity probably reflects protein degradation rather than specific de-acylation of the protein .
	manualset3
102738	6	400424	5	NULL	NULL	0	NULL	protein degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In pulse-chase experiments , the pattern of loss of the incorporated fatty acid was similar to that of the protein itself , and therefore the loss of radioactivity probably reflects protein degradation rather than specific de-acylation of the protein .
	manualset3
102739	7	400424	5	NULL	NULL	0	NULL	de-acylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In pulse-chase experiments , the pattern of loss of the incorporated fatty acid was similar to that of the protein itself , and therefore the loss of radioactivity probably reflects protein degradation rather than specific de-acylation of the protein .
	manualset3
102740	8	400424	5	NULL	NULL	0	NULL	protein 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In pulse-chase experiments , the pattern of loss of the incorporated fatty acid was similar to that of the protein itself , and therefore the loss of radioactivity probably reflects protein degradation rather than specific de-acylation of the protein .
	manualset3
102741	1	400425	5	NULL	NULL	0	NULL	quantitative analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In quantitative analysis , the TNR of PEM was significantly higher than that of PET/CT in the small-tumor groups , whereas no difference was found in the overall group .
	manualset3
102742	2	400425	5	NULL	NULL	0	NULL	TNR	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In quantitative analysis , the TNR of PEM was significantly higher than that of PET/CT in the small-tumor groups , whereas no difference was found in the overall group .
	manualset3
102743	3	400425	5	NULL	NULL	NULL	NULL	PEM	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In quantitative analysis , the TNR of PEM was significantly higher than that of PET/CT in the small-tumor groups , whereas no difference was found in the overall group .
	manualset3
102744	4	400425	5	NULL	NULL	0	NULL	PET/CT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In quantitative analysis , the TNR of PEM was significantly higher than that of PET/CT in the small-tumor groups , whereas no difference was found in the overall group .
	manualset3
102745	5	400425	5	NULL	NULL	0	NULL	small-tumor groups	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In quantitative analysis , the TNR of PEM was significantly higher than that of PET/CT in the small-tumor groups , whereas no difference was found in the overall group .
	manualset3
102746	6	400425	5	NULL	NULL	0	NULL	overall group	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In quantitative analysis , the TNR of PEM was significantly higher than that of PET/CT in the small-tumor groups , whereas no difference was found in the overall group .
	manualset3
109525	7	400425	5	NULL	NULL	0	NULL	difference	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In quantitative analysis , the TNR of PEM was significantly higher than that of PET/CT in the small-tumor groups , whereas no difference was found in the overall group .
	manualset3
102747	1	400426	5	NULL	NULL	0	NULL	rAN cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In rAN cells , ( ATP ) was increased in response to vibratory loading , attaining a level significantly greater than that of the control after 30 min of continuous vibration .
	manualset3
102748	2	400426	5	NULL	NULL	0	NULL	ATP 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In rAN cells , ( ATP ) was increased in response to vibratory loading , attaining a level significantly greater than that of the control after 30 min of continuous vibration .
	manualset3
102749	3	400426	5	NULL	NULL	0	NULL	response 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In rAN cells , ( ATP ) was increased in response to vibratory loading , attaining a level significantly greater than that of the control after 30 min of continuous vibration .
	manualset3
102751	4	400426	5	NULL	NULL	NULL	NULL	vibratory loading	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In rAN cells , ( ATP ) was increased in response to vibratory loading , attaining a level significantly greater than that of the control after 30 min of continuous vibration .
	manualset3
102752	5	400426	5	NULL	NULL	0	NULL	level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In rAN cells , ( ATP ) was increased in response to vibratory loading , attaining a level significantly greater than that of the control after 30 min of continuous vibration .
	manualset3
102753	6	400426	5	NULL	NULL	0	NULL	control	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In rAN cells , ( ATP ) was increased in response to vibratory loading , attaining a level significantly greater than that of the control after 30 min of continuous vibration .
	manualset3
102754	7	400426	5	NULL	NULL	0	NULL	30 min 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In rAN cells , ( ATP ) was increased in response to vibratory loading , attaining a level significantly greater than that of the control after 30 min of continuous vibration .
	manualset3
102755	8	400426	5	NULL	NULL	0	NULL	continuous vibration	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In rAN cells , ( ATP ) was increased in response to vibratory loading , attaining a level significantly greater than that of the control after 30 min of continuous vibration .
	manualset3
102756	1	400427	5	NULL	NULL	0	NULL	X-ray diffraction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	-- X-ray diffraction : crystallites in the acid-resistant specimens were larger by a factor of more than two .
	manualset3
102757	2	400427	5	NULL	NULL	0	NULL	crystallites	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	-- X-ray diffraction : crystallites in the acid-resistant specimens were larger by a factor of more than two .
	manualset3
102758	3	400427	5	NULL	NULL	0	NULL	acid-resistant specimens	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	-- X-ray diffraction : crystallites in the acid-resistant specimens were larger by a factor of more than two .
	manualset3
102760	4	400427	5	NULL	NULL	NULL	NULL	factor of more than two	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	-- X-ray diffraction : crystallites in the acid-resistant specimens were larger by a factor of more than two .
	manualset3
102762	1	400428	5	NULL	NULL	NULL	NULL	rare circumstances	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In rare circumstances , it is associated with familial syndromes , such as multiple endocrine neoplasia type 1 .
	manualset3
102764	2	400428	5	NULL	NULL	0	NULL	familial syndromes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In rare circumstances , it is associated with familial syndromes , such as multiple endocrine neoplasia type 1 .
	manualset3
102765	3	400428	5	NULL	NULL	0	NULL	multiple endocrine neoplasia type 1	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In rare circumstances , it is associated with familial syndromes , such as multiple endocrine neoplasia type 1 .
	manualset3
102774	1	400429	5	NULL	NULL	0	NULL	rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In rats fed a high fat diet ( HFD ) , long-term administration of 3 , 5-diiodo-L-thyronine ( T2 ) , a naturally occurring iodothyronine , was shown to reduce body-weight gain , fat mass , and hepatic lipid accumulation .
	manualset3
102775	2	400429	5	NULL	NULL	0	NULL	high fat diet ( HFD )	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	In rats fed a high fat diet ( HFD ) , long-term administration of 3 , 5-diiodo-L-thyronine ( T2 ) , a naturally occurring iodothyronine , was shown to reduce body-weight gain , fat mass , and hepatic lipid accumulation .
	manualset3
102776	3	400429	5	NULL	NULL	0	NULL	long-term administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In rats fed a high fat diet ( HFD ) , long-term administration of 3 , 5-diiodo-L-thyronine ( T2 ) , a naturally occurring iodothyronine , was shown to reduce body-weight gain , fat mass , and hepatic lipid accumulation .
	manualset3
102782	4	400429	5	NULL	NULL	0	NULL	3 , 5-diiodo-L-thyronine ( T2 ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In rats fed a high fat diet ( HFD ) , long-term administration of 3 , 5-diiodo-L-thyronine ( T2 ) , a naturally occurring iodothyronine , was shown to reduce body-weight gain , fat mass , and hepatic lipid accumulation .
	manualset3
102783	5	400429	5	NULL	NULL	0	NULL	naturally occurring iodothyronine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In rats fed a high fat diet ( HFD ) , long-term administration of 3 , 5-diiodo-L-thyronine ( T2 ) , a naturally occurring iodothyronine , was shown to reduce body-weight gain , fat mass , and hepatic lipid accumulation .
	manualset3
102784	6	400429	5	NULL	NULL	0	NULL	body-weight gain	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In rats fed a high fat diet ( HFD ) , long-term administration of 3 , 5-diiodo-L-thyronine ( T2 ) , a naturally occurring iodothyronine , was shown to reduce body-weight gain , fat mass , and hepatic lipid accumulation .
	manualset3
102786	7	400429	5	NULL	NULL	0	NULL	fat mass	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In rats fed a high fat diet ( HFD ) , long-term administration of 3 , 5-diiodo-L-thyronine ( T2 ) , a naturally occurring iodothyronine , was shown to reduce body-weight gain , fat mass , and hepatic lipid accumulation .
	manualset3
102788	8	400429	5	NULL	NULL	0	NULL	hepatic lipid accumulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In rats fed a high fat diet ( HFD ) , long-term administration of 3 , 5-diiodo-L-thyronine ( T2 ) , a naturally occurring iodothyronine , was shown to reduce body-weight gain , fat mass , and hepatic lipid accumulation .
	manualset3
102789	1	400430	5	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In rats with bile fistulas ( depletion model ) for 0.5 , 1 , 2 , 4 , and 7 days , both ntcp protein and mRNA expression remained unaltered .
	manualset3
102790	2	400430	5	NULL	NULL	0	NULL	bile fistulas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In rats with bile fistulas ( depletion model ) for 0.5 , 1 , 2 , 4 , and 7 days , both ntcp protein and mRNA expression remained unaltered .
	manualset3
102791	3	400430	5	NULL	NULL	0	NULL	depletion model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In rats with bile fistulas ( depletion model ) for 0.5 , 1 , 2 , 4 , and 7 days , both ntcp protein and mRNA expression remained unaltered .
	manualset3
102792	4	400430	5	NULL	NULL	0	NULL	0.5 , 1 , 2 , 4 , and 7 days	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In rats with bile fistulas ( depletion model ) for 0.5 , 1 , 2 , 4 , and 7 days , both ntcp protein and mRNA expression remained unaltered .
	manualset3
102793	5	400430	5	NULL	NULL	NULL	NULL	ntcp protein expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In rats with bile fistulas ( depletion model ) for 0.5 , 1 , 2 , 4 , and 7 days , both ntcp protein and mRNA expression remained unaltered .
	manualset3
102794	6	400430	5	NULL	NULL	0	NULL	ntcp mRNA expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In rats with bile fistulas ( depletion model ) for 0.5 , 1 , 2 , 4 , and 7 days , both ntcp protein and mRNA expression remained unaltered .
	manualset3
102856	1	400431	5	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In rats with renal failure , the plasma concentrations of 1 , 3-dimethyluric acid were considerably higher and the resultant AUC ( 0-6 h ) of 1 , 3-dimethyluric acid was significantly greater ( 44.4 vs 456 microg min mL ( -1 ) ) compared with control rats .
	manualset3
102872	2	400431	5	NULL	NULL	0	NULL	renal failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In rats with renal failure , the plasma concentrations of 1 , 3-dimethyluric acid were considerably higher and the resultant AUC ( 0-6 h ) of 1 , 3-dimethyluric acid was significantly greater ( 44.4 vs 456 microg min mL ( -1 ) ) compared with control rats .
	manualset3
102873	3	400431	5	NULL	NULL	0	NULL	plasma concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In rats with renal failure , the plasma concentrations of 1 , 3-dimethyluric acid were considerably higher and the resultant AUC ( 0-6 h ) of 1 , 3-dimethyluric acid was significantly greater ( 44.4 vs 456 microg min mL ( -1 ) ) compared with control rats .
	manualset3
102874	4	400431	5	NULL	NULL	0	NULL	1 , 3-dimethyluric acid	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In rats with renal failure , the plasma concentrations of 1 , 3-dimethyluric acid were considerably higher and the resultant AUC ( 0-6 h ) of 1 , 3-dimethyluric acid was significantly greater ( 44.4 vs 456 microg min mL ( -1 ) ) compared with control rats .
	manualset3
102875	5	400431	5	NULL	NULL	0	NULL	AUC	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In rats with renal failure , the plasma concentrations of 1 , 3-dimethyluric acid were considerably higher and the resultant AUC ( 0-6 h ) of 1 , 3-dimethyluric acid was significantly greater ( 44.4 vs 456 microg min mL ( -1 ) ) compared with control rats .
	manualset3
102876	6	400431	5	NULL	NULL	0	NULL	0-6 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In rats with renal failure , the plasma concentrations of 1 , 3-dimethyluric acid were considerably higher and the resultant AUC ( 0-6 h ) of 1 , 3-dimethyluric acid was significantly greater ( 44.4 vs 456 microg min mL ( -1 ) ) compared with control rats .
	manualset3
102877	7	400431	5	NULL	NULL	0	NULL	1 , 3-dimethyluric acid	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In rats with renal failure , the plasma concentrations of 1 , 3-dimethyluric acid were considerably higher and the resultant AUC ( 0-6 h ) of 1 , 3-dimethyluric acid was significantly greater ( 44.4 vs 456 microg min mL ( -1 ) ) compared with control rats .
	manualset3
102878	8	400431	5	NULL	NULL	0	NULL	44.4 vs 456 microg min mL ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In rats with renal failure , the plasma concentrations of 1 , 3-dimethyluric acid were considerably higher and the resultant AUC ( 0-6 h ) of 1 , 3-dimethyluric acid was significantly greater ( 44.4 vs 456 microg min mL ( -1 ) ) compared with control rats .
	manualset3
102884	9	400431	5	NULL	NULL	0	NULL	control rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In rats with renal failure , the plasma concentrations of 1 , 3-dimethyluric acid were considerably higher and the resultant AUC ( 0-6 h ) of 1 , 3-dimethyluric acid was significantly greater ( 44.4 vs 456 microg min mL ( -1 ) ) compared with control rats .
	manualset3
103069	1	400432	5	NULL	NULL	0	NULL	recent decades	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent decades growing evidence has accumulated on the hormone-like effects of synthetic chemicals that appeared in the environment .
	manualset3
103070	2	400432	5	NULL	NULL	0	NULL	growing evidence	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent decades growing evidence has accumulated on the hormone-like effects of synthetic chemicals that appeared in the environment .
	manualset3
103071	3	400432	5	NULL	NULL	0	NULL	hormone-like effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent decades growing evidence has accumulated on the hormone-like effects of synthetic chemicals that appeared in the environment .
	manualset3
103072	4	400432	5	NULL	NULL	0	NULL	synthetic chemicals	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent decades growing evidence has accumulated on the hormone-like effects of synthetic chemicals that appeared in the environment .
	manualset3
103073	5	400432	5	NULL	NULL	0	NULL	environment	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent decades growing evidence has accumulated on the hormone-like effects of synthetic chemicals that appeared in the environment .
	manualset3
103074	1	400433	5	NULL	NULL	0	NULL	recent years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years , interfacial properties have been tailored with nanostructured polymer assemblies to generate materials with specific properties and functions for application in diverse fields , including biomaterials , drug delivery , catalysis , sensing , optics and corrosion .
	manualset3
103075	2	400433	5	NULL	NULL	0	NULL	interfacial properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years , interfacial properties have been tailored with nanostructured polymer assemblies to generate materials with specific properties and functions for application in diverse fields , including biomaterials , drug delivery , catalysis , sensing , optics and corrosion .
	manualset3
103076	3	400433	5	NULL	NULL	NULL	NULL	nanostructured polymer assemblies	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In recent years , interfacial properties have been tailored with nanostructured polymer assemblies to generate materials with specific properties and functions for application in diverse fields , including biomaterials , drug delivery , catalysis , sensing , optics and corrosion .
	manualset3
103077	4	400433	5	NULL	NULL	0	NULL	materials	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years , interfacial properties have been tailored with nanostructured polymer assemblies to generate materials with specific properties and functions for application in diverse fields , including biomaterials , drug delivery , catalysis , sensing , optics and corrosion .
	manualset3
103078	5	400433	5	NULL	NULL	0	NULL	specific properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years , interfacial properties have been tailored with nanostructured polymer assemblies to generate materials with specific properties and functions for application in diverse fields , including biomaterials , drug delivery , catalysis , sensing , optics and corrosion .
	manualset3
103082	6	400433	5	NULL	NULL	0	NULL	functions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years , interfacial properties have been tailored with nanostructured polymer assemblies to generate materials with specific properties and functions for application in diverse fields , including biomaterials , drug delivery , catalysis , sensing , optics and corrosion .
	manualset3
103083	7	400433	5	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years , interfacial properties have been tailored with nanostructured polymer assemblies to generate materials with specific properties and functions for application in diverse fields , including biomaterials , drug delivery , catalysis , sensing , optics and corrosion .
	manualset3
103084	8	400433	5	NULL	NULL	0	NULL	diverse fields	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years , interfacial properties have been tailored with nanostructured polymer assemblies to generate materials with specific properties and functions for application in diverse fields , including biomaterials , drug delivery , catalysis , sensing , optics and corrosion .
	manualset3
103085	9	400433	5	NULL	NULL	0	NULL	biomaterials	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years , interfacial properties have been tailored with nanostructured polymer assemblies to generate materials with specific properties and functions for application in diverse fields , including biomaterials , drug delivery , catalysis , sensing , optics and corrosion .
	manualset3
103086	10	400433	5	NULL	NULL	0	NULL	drug delivery	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years , interfacial properties have been tailored with nanostructured polymer assemblies to generate materials with specific properties and functions for application in diverse fields , including biomaterials , drug delivery , catalysis , sensing , optics and corrosion .
	manualset3
103087	11	400433	5	NULL	NULL	0	NULL	catalysis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years , interfacial properties have been tailored with nanostructured polymer assemblies to generate materials with specific properties and functions for application in diverse fields , including biomaterials , drug delivery , catalysis , sensing , optics and corrosion .
	manualset3
103088	12	400433	5	NULL	NULL	0	NULL	sensing 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years , interfacial properties have been tailored with nanostructured polymer assemblies to generate materials with specific properties and functions for application in diverse fields , including biomaterials , drug delivery , catalysis , sensing , optics and corrosion .
	manualset3
103089	13	400433	5	NULL	NULL	0	NULL	optics 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years , interfacial properties have been tailored with nanostructured polymer assemblies to generate materials with specific properties and functions for application in diverse fields , including biomaterials , drug delivery , catalysis , sensing , optics and corrosion .
	manualset3
103090	14	400433	5	NULL	NULL	0	NULL	corrosion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years , interfacial properties have been tailored with nanostructured polymer assemblies to generate materials with specific properties and functions for application in diverse fields , including biomaterials , drug delivery , catalysis , sensing , optics and corrosion .
	manualset3
103091	1	400434	5	NULL	NULL	0	NULL	recent years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years , the MML action plan has funded many projects designed to bring about a rapprochement between science ( and scientists ) and other civil society actors .
	manualset3
103092	2	400434	5	NULL	NULL	0	NULL	MML action plan	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years , the MML action plan has funded many projects designed to bring about a rapprochement between science ( and scientists ) and other civil society actors .
	manualset3
103093	3	400434	5	NULL	NULL	0	NULL	projects	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years , the MML action plan has funded many projects designed to bring about a rapprochement between science ( and scientists ) and other civil society actors .
	manualset3
103094	4	400434	5	NULL	NULL	0	NULL	rapprochement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years , the MML action plan has funded many projects designed to bring about a rapprochement between science ( and scientists ) and other civil society actors .
	manualset3
103095	5	400434	5	NULL	NULL	0	NULL	science	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years , the MML action plan has funded many projects designed to bring about a rapprochement between science ( and scientists ) and other civil society actors .
	manualset3
103096	6	400434	5	NULL	NULL	0	NULL	scientists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years , the MML action plan has funded many projects designed to bring about a rapprochement between science ( and scientists ) and other civil society actors .
	manualset3
103097	7	400434	5	NULL	NULL	0	NULL	civil society actors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years , the MML action plan has funded many projects designed to bring about a rapprochement between science ( and scientists ) and other civil society actors .
	manualset3
103098	1	400435	5	NULL	NULL	0	NULL	( Z , Z ) -15 - hydroxy-7 , 7 - dimethyl-5 , 8 - eicosadienoic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	- ( Z , Z ) -15 - hydroxy-7 , 7 - dimethyl-5 , 8 - eicosadienoic acid are described .
	manualset3
103099	1	400436	5	NULL	NULL	0	NULL	recent years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years an increased risk of male breast cancer has been reported in families with positive family history and in which BRCA2 mutations have been identified .
	manualset3
103100	2	400436	5	NULL	NULL	0	NULL	increased risk	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years an increased risk of male breast cancer has been reported in families with positive family history and in which BRCA2 mutations have been identified .
	manualset3
103101	3	400436	5	NULL	NULL	0	NULL	male breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years an increased risk of male breast cancer has been reported in families with positive family history and in which BRCA2 mutations have been identified .
	manualset3
103102	4	400436	5	NULL	NULL	0	NULL	families 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years an increased risk of male breast cancer has been reported in families with positive family history and in which BRCA2 mutations have been identified .
	manualset3
103103	5	400436	5	NULL	NULL	0	NULL	positive family history	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years an increased risk of male breast cancer has been reported in families with positive family history and in which BRCA2 mutations have been identified .
	manualset3
103104	6	400436	5	NULL	NULL	0	NULL	BRCA2 mutations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years an increased risk of male breast cancer has been reported in families with positive family history and in which BRCA2 mutations have been identified .
	manualset3
103105	1	400437	5	NULL	NULL	0	NULL	recent years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years it has become evident that secretion of saliva may not be elicited only by cholinergic or adrenergic agonists but also by peptides , injected into the bloodstream , and further , that the salivary secretion in response to stimulation of the parasympathetic innervation is not always completely abolished by the muscarinic receptor blocker atropine ( and adrenoceptor antagonists ) .
	manualset3
103106	2	400437	5	NULL	NULL	0	NULL	secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years it has become evident that secretion of saliva may not be elicited only by cholinergic or adrenergic agonists but also by peptides , injected into the bloodstream , and further , that the salivary secretion in response to stimulation of the parasympathetic innervation is not always completely abolished by the muscarinic receptor blocker atropine ( and adrenoceptor antagonists ) .
	manualset3
103107	3	400437	5	NULL	NULL	0	NULL	saliva	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years it has become evident that secretion of saliva may not be elicited only by cholinergic or adrenergic agonists but also by peptides , injected into the bloodstream , and further , that the salivary secretion in response to stimulation of the parasympathetic innervation is not always completely abolished by the muscarinic receptor blocker atropine ( and adrenoceptor antagonists ) .
	manualset3
103108	4	400437	5	NULL	NULL	0	NULL	cholinergic or adrenergic agonists	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years it has become evident that secretion of saliva may not be elicited only by cholinergic or adrenergic agonists but also by peptides , injected into the bloodstream , and further , that the salivary secretion in response to stimulation of the parasympathetic innervation is not always completely abolished by the muscarinic receptor blocker atropine ( and adrenoceptor antagonists ) .
	manualset3
103109	5	400437	5	NULL	NULL	NULL	NULL	peptides	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In recent years it has become evident that secretion of saliva may not be elicited only by cholinergic or adrenergic agonists but also by peptides , injected into the bloodstream , and further , that the salivary secretion in response to stimulation of the parasympathetic innervation is not always completely abolished by the muscarinic receptor blocker atropine ( and adrenoceptor antagonists ) .
	manualset3
103110	6	400437	5	NULL	NULL	0	NULL	bloodstream	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years it has become evident that secretion of saliva may not be elicited only by cholinergic or adrenergic agonists but also by peptides , injected into the bloodstream , and further , that the salivary secretion in response to stimulation of the parasympathetic innervation is not always completely abolished by the muscarinic receptor blocker atropine ( and adrenoceptor antagonists ) .
	manualset3
103111	7	400437	5	NULL	NULL	0	NULL	salivary secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years it has become evident that secretion of saliva may not be elicited only by cholinergic or adrenergic agonists but also by peptides , injected into the bloodstream , and further , that the salivary secretion in response to stimulation of the parasympathetic innervation is not always completely abolished by the muscarinic receptor blocker atropine ( and adrenoceptor antagonists ) .
	manualset3
103112	8	400437	5	NULL	NULL	0	NULL	response to stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years it has become evident that secretion of saliva may not be elicited only by cholinergic or adrenergic agonists but also by peptides , injected into the bloodstream , and further , that the salivary secretion in response to stimulation of the parasympathetic innervation is not always completely abolished by the muscarinic receptor blocker atropine ( and adrenoceptor antagonists ) .
	manualset3
103113	9	400437	5	NULL	NULL	0	NULL	parasympathetic innervation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years it has become evident that secretion of saliva may not be elicited only by cholinergic or adrenergic agonists but also by peptides , injected into the bloodstream , and further , that the salivary secretion in response to stimulation of the parasympathetic innervation is not always completely abolished by the muscarinic receptor blocker atropine ( and adrenoceptor antagonists ) .
	manualset3
103114	10	400437	5	NULL	NULL	0	NULL	muscarinic receptor blocker atropine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years it has become evident that secretion of saliva may not be elicited only by cholinergic or adrenergic agonists but also by peptides , injected into the bloodstream , and further , that the salivary secretion in response to stimulation of the parasympathetic innervation is not always completely abolished by the muscarinic receptor blocker atropine ( and adrenoceptor antagonists ) .
	manualset3
103115	11	400437	5	NULL	NULL	0	NULL	adrenoceptor antagonists	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years it has become evident that secretion of saliva may not be elicited only by cholinergic or adrenergic agonists but also by peptides , injected into the bloodstream , and further , that the salivary secretion in response to stimulation of the parasympathetic innervation is not always completely abolished by the muscarinic receptor blocker atropine ( and adrenoceptor antagonists ) .
	manualset3
103116	1	400438	5	NULL	NULL	0	NULL	recent years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years there has been an increase in the number of users of nonisotopic automated methods ( Abbott TDx mono , AxSYM , Dade-Behring EMIT or Microgenic Cedia ) , which render instantaneous analysis possible .
	manualset3
103117	2	400438	5	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years there has been an increase in the number of users of nonisotopic automated methods ( Abbott TDx mono , AxSYM , Dade-Behring EMIT or Microgenic Cedia ) , which render instantaneous analysis possible .
	manualset3
103118	3	400438	5	NULL	NULL	0	NULL	users 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years there has been an increase in the number of users of nonisotopic automated methods ( Abbott TDx mono , AxSYM , Dade-Behring EMIT or Microgenic Cedia ) , which render instantaneous analysis possible .
	manualset3
103119	4	400438	5	NULL	NULL	0	NULL	nonisotopic automated methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years there has been an increase in the number of users of nonisotopic automated methods ( Abbott TDx mono , AxSYM , Dade-Behring EMIT or Microgenic Cedia ) , which render instantaneous analysis possible .
	manualset3
103120	5	400438	5	NULL	NULL	NULL	NULL	Abbott TDx mono	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In recent years there has been an increase in the number of users of nonisotopic automated methods ( Abbott TDx mono , AxSYM , Dade-Behring EMIT or Microgenic Cedia ) , which render instantaneous analysis possible .
	manualset3
103121	6	400438	5	NULL	NULL	0	NULL	AxSYM 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years there has been an increase in the number of users of nonisotopic automated methods ( Abbott TDx mono , AxSYM , Dade-Behring EMIT or Microgenic Cedia ) , which render instantaneous analysis possible .
	manualset3
103122	7	400438	5	NULL	NULL	0	NULL	Dade-Behring EMIT	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years there has been an increase in the number of users of nonisotopic automated methods ( Abbott TDx mono , AxSYM , Dade-Behring EMIT or Microgenic Cedia ) , which render instantaneous analysis possible .
	manualset3
103123	8	400438	5	NULL	NULL	0	NULL	Microgenic Cedia	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years there has been an increase in the number of users of nonisotopic automated methods ( Abbott TDx mono , AxSYM , Dade-Behring EMIT or Microgenic Cedia ) , which render instantaneous analysis possible .
	manualset3
107680	9	400438	5	NULL	NULL	0	NULL	render instantaneous analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In recent years there has been an increase in the number of users of nonisotopic automated methods ( Abbott TDx mono , AxSYM , Dade-Behring EMIT or Microgenic Cedia ) , which render instantaneous analysis possible .
	manualset3
103124	1	400439	5	NULL	NULL	0	NULL	regime VVI	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In regime VVI both SAP and DAP lowering was more pronounced than in AAI regime .
	manualset3
103125	2	400439	5	NULL	NULL	0	NULL	SAP	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In regime VVI both SAP and DAP lowering was more pronounced than in AAI regime .
	manualset3
103126	3	400439	5	NULL	NULL	0	NULL	DAP	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In regime VVI both SAP and DAP lowering was more pronounced than in AAI regime .
	manualset3
103127	4	400439	5	NULL	NULL	0	NULL	AAI regime 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In regime VVI both SAP and DAP lowering was more pronounced than in AAI regime .
	manualset3
103128	1	400440	5	NULL	NULL	0	NULL	day 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In relation to the day of the first successful insemination , we recorded a significant increase in T4 concentration ( P less than 0.001 ; P less than 0.001 ) on the day of the second , or third successful inseminations .
	manualset3
103129	2	400440	5	NULL	NULL	NULL	NULL	first successful insemination	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In relation to the day of the first successful insemination , we recorded a significant increase in T4 concentration ( P less than 0.001 ; P less than 0.001 ) on the day of the second , or third successful inseminations .
	manualset3
103130	3	400440	5	NULL	NULL	0	NULL	T4 concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In relation to the day of the first successful insemination , we recorded a significant increase in T4 concentration ( P less than 0.001 ; P less than 0.001 ) on the day of the second , or third successful inseminations .
	manualset3
103131	4	400440	5	NULL	NULL	0	NULL	P less than 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In relation to the day of the first successful insemination , we recorded a significant increase in T4 concentration ( P less than 0.001 ; P less than 0.001 ) on the day of the second , or third successful inseminations .
	manualset3
103132	5	400440	5	NULL	NULL	0	NULL	P less than 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In relation to the day of the first successful insemination , we recorded a significant increase in T4 concentration ( P less than 0.001 ; P less than 0.001 ) on the day of the second , or third successful inseminations .
	manualset3
103133	6	400440	5	NULL	NULL	0	NULL	day	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In relation to the day of the first successful insemination , we recorded a significant increase in T4 concentration ( P less than 0.001 ; P less than 0.001 ) on the day of the second , or third successful inseminations .
	manualset3
103134	7	400440	5	NULL	NULL	0	NULL	second , or third successful inseminations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In relation to the day of the first successful insemination , we recorded a significant increase in T4 concentration ( P less than 0.001 ; P less than 0.001 ) on the day of the second , or third successful inseminations .
	manualset3
103135	1	400441	5	NULL	NULL	0	NULL	endurance exercise 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In response to endurance exercise , the superoxide dismutase activity markedly decreased in sedentary control subjects .
	manualset3
103136	2	400441	5	NULL	NULL	0	NULL	superoxide dismutase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In response to endurance exercise , the superoxide dismutase activity markedly decreased in sedentary control subjects .
	manualset3
103137	3	400441	5	NULL	NULL	0	NULL	sedentary control subjects	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In response to endurance exercise , the superoxide dismutase activity markedly decreased in sedentary control subjects .
	manualset3
103138	1	400442	5	NULL	NULL	0	NULL	hydrophobicity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In response to hydrophobicity and hydroxy fatty acids , U. maydis develops infection structures called appressoria .
	manualset3
103139	2	400442	5	NULL	NULL	0	NULL	hydroxy fatty acids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In response to hydrophobicity and hydroxy fatty acids , U. maydis develops infection structures called appressoria .
	manualset3
103140	3	400442	5	NULL	NULL	0	NULL	U. maydis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In response to hydrophobicity and hydroxy fatty acids , U. maydis develops infection structures called appressoria .
	manualset3
103141	4	400442	5	NULL	NULL	0	NULL	infection structures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In response to hydrophobicity and hydroxy fatty acids , U. maydis develops infection structures called appressoria .
	manualset3
103142	5	400442	5	NULL	NULL	0	NULL	appressoria	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In response to hydrophobicity and hydroxy fatty acids , U. maydis develops infection structures called appressoria .
	manualset3
103143	1	400443	5	NULL	NULL	0	NULL	resistance training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In response to resistance training , TEE increased and RER decreased .
	manualset3
103144	2	400443	5	NULL	NULL	NULL	NULL	TEE	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In response to resistance training , TEE increased and RER decreased .
	manualset3
103145	3	400443	5	NULL	NULL	0	NULL	RER	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In response to resistance training , TEE increased and RER decreased .
	manualset3
103146	1	400444	5	NULL	NULL	0	NULL	dependent mechanism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	- ) - dependent mechanism that requires L-cystine and redox-active transition metal ions in the incubation medium .
	manualset3
103147	2	400444	5	NULL	NULL	0	NULL	L-cystine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	- ) - dependent mechanism that requires L-cystine and redox-active transition metal ions in the incubation medium .
	manualset3
103148	3	400444	5	NULL	NULL	0	NULL	redox-active transition metal ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	- ) - dependent mechanism that requires L-cystine and redox-active transition metal ions in the incubation medium .
	manualset3
103149	4	400444	5	NULL	NULL	0	NULL	incubation medium	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	- ) - dependent mechanism that requires L-cystine and redox-active transition metal ions in the incubation medium .
	manualset3
103150	1	400445	5	NULL	NULL	0	NULL	sinusoidal potential changes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In response to sinusoidal potential changes a 1 : 1 relation between each afferent impulse and the peak of the stimulating waveform could be obtained over the range 12-300 Hz .
	manualset3
103151	2	400445	5	NULL	NULL	0	NULL	1 : 1 relation	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In response to sinusoidal potential changes a 1 : 1 relation between each afferent impulse and the peak of the stimulating waveform could be obtained over the range 12-300 Hz .
	manualset3
103152	3	400445	5	NULL	NULL	0	NULL	afferent impulse	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In response to sinusoidal potential changes a 1 : 1 relation between each afferent impulse and the peak of the stimulating waveform could be obtained over the range 12-300 Hz .
	manualset3
103153	4	400445	5	NULL	NULL	0	NULL	peak of the stimulating waveform	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In response to sinusoidal potential changes a 1 : 1 relation between each afferent impulse and the peak of the stimulating waveform could be obtained over the range 12-300 Hz .
	manualset3
103154	5	400445	5	NULL	NULL	0	NULL	range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In response to sinusoidal potential changes a 1 : 1 relation between each afferent impulse and the peak of the stimulating waveform could be obtained over the range 12-300 Hz .
	manualset3
103155	6	400445	5	NULL	NULL	0	NULL	12-300 Hz	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In response to sinusoidal potential changes a 1 : 1 relation between each afferent impulse and the peak of the stimulating waveform could be obtained over the range 12-300 Hz .
	manualset3
103156	1	400446	5	NULL	NULL	0	NULL	round spermatids	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In round spermatids , essentially all of MP1-mRNA is 580 bases long and is in the nonpolysomal fraction .
	manualset3
103157	2	400446	5	NULL	NULL	0	NULL	MP1-mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In round spermatids , essentially all of MP1-mRNA is 580 bases long and is in the nonpolysomal fraction .
	manualset3
103158	3	400446	5	NULL	NULL	0	NULL	580 bases	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In round spermatids , essentially all of MP1-mRNA is 580 bases long and is in the nonpolysomal fraction .
	manualset3
103159	4	400446	5	NULL	NULL	0	NULL	nonpolysomal fraction	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In round spermatids , essentially all of MP1-mRNA is 580 bases long and is in the nonpolysomal fraction .
	manualset3
103160	1	400447	5	NULL	NULL	0	NULL	fraction	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In search for the unaccounted for fraction of the ( 14 ) C-quercetin dose , we performed ( 14 ) CO ( 2 ) recovery studies in three volunteers ( 3 iv and 3 oral doses ) .
	manualset3
103161	2	400447	5	NULL	NULL	0	NULL	( 14 ) C-quercetin dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In search for the unaccounted for fraction of the ( 14 ) C-quercetin dose , we performed ( 14 ) CO ( 2 ) recovery studies in three volunteers ( 3 iv and 3 oral doses ) .
	manualset3
103162	3	400447	5	NULL	NULL	0	NULL	( 14 ) CO ( 2 )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In search for the unaccounted for fraction of the ( 14 ) C-quercetin dose , we performed ( 14 ) CO ( 2 ) recovery studies in three volunteers ( 3 iv and 3 oral doses ) .
	manualset3
103163	4	400447	5	NULL	NULL	0	NULL	recovery studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In search for the unaccounted for fraction of the ( 14 ) C-quercetin dose , we performed ( 14 ) CO ( 2 ) recovery studies in three volunteers ( 3 iv and 3 oral doses ) .
	manualset3
103164	5	400447	5	NULL	NULL	0	NULL	three volunteers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In search for the unaccounted for fraction of the ( 14 ) C-quercetin dose , we performed ( 14 ) CO ( 2 ) recovery studies in three volunteers ( 3 iv and 3 oral doses ) .
	manualset3
103165	6	400447	5	NULL	NULL	0	NULL	3 iv	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In search for the unaccounted for fraction of the ( 14 ) C-quercetin dose , we performed ( 14 ) CO ( 2 ) recovery studies in three volunteers ( 3 iv and 3 oral doses ) .
	manualset3
103166	7	400447	5	NULL	NULL	0	NULL	3 oral doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In search for the unaccounted for fraction of the ( 14 ) C-quercetin dose , we performed ( 14 ) CO ( 2 ) recovery studies in three volunteers ( 3 iv and 3 oral doses ) .
	manualset3
103167	1	400448	5	NULL	NULL	0	NULL	safer myelographic technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In search of a safer myelographic technique , we performed myelography via the lumbosacral intervertebral space .
	manualset3
103168	2	400448	5	NULL	NULL	0	NULL	myelography 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In search of a safer myelographic technique , we performed myelography via the lumbosacral intervertebral space .
	manualset3
103169	3	400448	5	NULL	NULL	0	NULL	lumbosacral intervertebral space	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In search of a safer myelographic technique , we performed myelography via the lumbosacral intervertebral space .
	manualset3
103170	1	400449	5	NULL	NULL	0	NULL	hot appendix	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In search of the hot appendix -- a clinician 's view of inflammation imaging .
	manualset3
103171	2	400449	5	NULL	NULL	0	NULL	clinician 's view	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In search of the hot appendix -- a clinician 's view of inflammation imaging .
	manualset3
103172	3	400449	5	NULL	NULL	0	NULL	inflammation imaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In search of the hot appendix -- a clinician 's view of inflammation imaging .
	manualset3
103173	1	400450	5	NULL	NULL	0	NULL	seminiferous tubules	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In seminiferous tubules with normal spermatogenesis , Cx43 expression was found between Sertoli cells and germ cells .
	manualset3
103174	2	400450	5	NULL	NULL	0	NULL	normal spermatogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In seminiferous tubules with normal spermatogenesis , Cx43 expression was found between Sertoli cells and germ cells .
	manualset3
103175	3	400450	5	NULL	NULL	0	NULL	Cx43 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In seminiferous tubules with normal spermatogenesis , Cx43 expression was found between Sertoli cells and germ cells .
	manualset3
103176	4	400450	5	NULL	NULL	0	NULL	Sertoli cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In seminiferous tubules with normal spermatogenesis , Cx43 expression was found between Sertoli cells and germ cells .
	manualset3
103177	5	400450	5	NULL	NULL	0	NULL	germ cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In seminiferous tubules with normal spermatogenesis , Cx43 expression was found between Sertoli cells and germ cells .
	manualset3
103218	1	400451	5	NULL	NULL	0	NULL	senile dementia of the Alzheimer type	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In senile dementia of the Alzheimer type , a striking increase in the frequency of the rare C4B locus allele , C4 * B2 , was apparent , resulting in the high relative risk of RR = 8.8 ( p less than 0.0001 ) for this disorder .
	manualset3
103219	2	400451	5	NULL	NULL	0	NULL	frequency 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In senile dementia of the Alzheimer type , a striking increase in the frequency of the rare C4B locus allele , C4 * B2 , was apparent , resulting in the high relative risk of RR = 8.8 ( p less than 0.0001 ) for this disorder .
	manualset3
103220	3	400451	5	NULL	NULL	NULL	NULL	C4B locus allele , C4 * B2	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In senile dementia of the Alzheimer type , a striking increase in the frequency of the rare C4B locus allele , C4 * B2 , was apparent , resulting in the high relative risk of RR = 8.8 ( p less than 0.0001 ) for this disorder .
	manualset3
103221	4	400451	5	NULL	NULL	0	NULL	high relative risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In senile dementia of the Alzheimer type , a striking increase in the frequency of the rare C4B locus allele , C4 * B2 , was apparent , resulting in the high relative risk of RR = 8.8 ( p less than 0.0001 ) for this disorder .
	manualset3
103222	5	400451	5	NULL	NULL	0	NULL	RR = 8.8	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In senile dementia of the Alzheimer type , a striking increase in the frequency of the rare C4B locus allele , C4 * B2 , was apparent , resulting in the high relative risk of RR = 8.8 ( p less than 0.0001 ) for this disorder .
	manualset3
103223	6	400451	5	NULL	NULL	0	NULL	p less than 0.0001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In senile dementia of the Alzheimer type , a striking increase in the frequency of the rare C4B locus allele , C4 * B2 , was apparent , resulting in the high relative risk of RR = 8.8 ( p less than 0.0001 ) for this disorder .
	manualset3
103224	7	400451	5	NULL	NULL	0	NULL	disorder 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In senile dementia of the Alzheimer type , a striking increase in the frequency of the rare C4B locus allele , C4 * B2 , was apparent , resulting in the high relative risk of RR = 8.8 ( p less than 0.0001 ) for this disorder .
	manualset3
103225	1	400452	5	NULL	NULL	0	NULL	septic aorta	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In septic aorta , total and surface expression levels of the two death receptors tumor necrosis factor receptor 1 and Fas were highly upregulated .
	manualset3
103226	2	400452	5	NULL	NULL	0	NULL	total and surface expression levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In septic aorta , total and surface expression levels of the two death receptors tumor necrosis factor receptor 1 and Fas were highly upregulated .
	manualset3
103227	3	400452	5	NULL	NULL	0	NULL	two death receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In septic aorta , total and surface expression levels of the two death receptors tumor necrosis factor receptor 1 and Fas were highly upregulated .
	manualset3
103228	4	400452	5	NULL	NULL	0	NULL	tumor necrosis factor receptor 1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In septic aorta , total and surface expression levels of the two death receptors tumor necrosis factor receptor 1 and Fas were highly upregulated .
	manualset3
103229	5	400452	5	NULL	NULL	0	NULL	Fas	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In septic aorta , total and surface expression levels of the two death receptors tumor necrosis factor receptor 1 and Fas were highly upregulated .
	manualset3
103230	1	400453	5	NULL	NULL	NULL	NULL	seven Swedish foundries	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In seven Swedish foundries and two remelting plants , the exposure and area concentrations of total dust , metals , organic gases , and vapors were determined mainly as daily , time-weighted averages ( TWAs ) .
	manualset3
103231	2	400453	5	NULL	NULL	0	NULL	remelting plants	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In seven Swedish foundries and two remelting plants , the exposure and area concentrations of total dust , metals , organic gases , and vapors were determined mainly as daily , time-weighted averages ( TWAs ) .
	manualset3
103232	3	400453	5	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In seven Swedish foundries and two remelting plants , the exposure and area concentrations of total dust , metals , organic gases , and vapors were determined mainly as daily , time-weighted averages ( TWAs ) .
	manualset3
103233	4	400453	5	NULL	NULL	0	NULL	area concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In seven Swedish foundries and two remelting plants , the exposure and area concentrations of total dust , metals , organic gases , and vapors were determined mainly as daily , time-weighted averages ( TWAs ) .
	manualset3
103234	5	400453	5	NULL	NULL	0	NULL	total dust	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In seven Swedish foundries and two remelting plants , the exposure and area concentrations of total dust , metals , organic gases , and vapors were determined mainly as daily , time-weighted averages ( TWAs ) .
	manualset3
103235	6	400453	5	NULL	NULL	0	NULL	metals	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In seven Swedish foundries and two remelting plants , the exposure and area concentrations of total dust , metals , organic gases , and vapors were determined mainly as daily , time-weighted averages ( TWAs ) .
	manualset3
103236	7	400453	5	NULL	NULL	0	NULL	organic gases	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In seven Swedish foundries and two remelting plants , the exposure and area concentrations of total dust , metals , organic gases , and vapors were determined mainly as daily , time-weighted averages ( TWAs ) .
	manualset3
103237	8	400453	5	NULL	NULL	0	NULL	vapors	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In seven Swedish foundries and two remelting plants , the exposure and area concentrations of total dust , metals , organic gases , and vapors were determined mainly as daily , time-weighted averages ( TWAs ) .
	manualset3
103238	9	400453	5	NULL	NULL	0	NULL	daily	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In seven Swedish foundries and two remelting plants , the exposure and area concentrations of total dust , metals , organic gases , and vapors were determined mainly as daily , time-weighted averages ( TWAs ) .
	manualset3
103239	10	400453	5	NULL	NULL	0	NULL	time-weighted averages ( TWAs )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In seven Swedish foundries and two remelting plants , the exposure and area concentrations of total dust , metals , organic gases , and vapors were determined mainly as daily , time-weighted averages ( TWAs ) .
	manualset3
103240	1	400454	5	NULL	NULL	0	NULL	short-term tissue cultures	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In short-term tissue cultures dibutyryl cAMP inhibits the cortisone-induced degranulation of mast cells .
	manualset3
103241	2	400454	5	NULL	NULL	0	NULL	dibutyryl cAMP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In short-term tissue cultures dibutyryl cAMP inhibits the cortisone-induced degranulation of mast cells .
	manualset3
103242	3	400454	5	NULL	NULL	0	NULL	cortisone-induced degranulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In short-term tissue cultures dibutyryl cAMP inhibits the cortisone-induced degranulation of mast cells .
	manualset3
103243	4	400454	5	NULL	NULL	0	NULL	mast cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In short-term tissue cultures dibutyryl cAMP inhibits the cortisone-induced degranulation of mast cells .
	manualset3
103244	1	400455	5	NULL	NULL	0	NULL	six complete moles	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In six complete moles the mtDNA was found to be maternal in origin , with no contribution from the sperm mitochondria , while the nuclear genome was shown to be exclusively paternal in five cases .
	manualset3
103245	2	400455	5	NULL	NULL	0	NULL	mtDNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In six complete moles the mtDNA was found to be maternal in origin , with no contribution from the sperm mitochondria , while the nuclear genome was shown to be exclusively paternal in five cases .
	manualset3
103246	3	400455	5	NULL	NULL	0	NULL	origin	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In six complete moles the mtDNA was found to be maternal in origin , with no contribution from the sperm mitochondria , while the nuclear genome was shown to be exclusively paternal in five cases .
	manualset3
103247	4	400455	5	NULL	NULL	0	NULL	contribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In six complete moles the mtDNA was found to be maternal in origin , with no contribution from the sperm mitochondria , while the nuclear genome was shown to be exclusively paternal in five cases .
	manualset3
103248	5	400455	5	NULL	NULL	0	NULL	sperm mitochondria	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In six complete moles the mtDNA was found to be maternal in origin , with no contribution from the sperm mitochondria , while the nuclear genome was shown to be exclusively paternal in five cases .
	manualset3
103249	6	400455	5	NULL	NULL	0	NULL	nuclear genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In six complete moles the mtDNA was found to be maternal in origin , with no contribution from the sperm mitochondria , while the nuclear genome was shown to be exclusively paternal in five cases .
	manualset3
103250	7	400455	5	NULL	NULL	0	NULL	five cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In six complete moles the mtDNA was found to be maternal in origin , with no contribution from the sperm mitochondria , while the nuclear genome was shown to be exclusively paternal in five cases .
	manualset3
103251	1	400456	5	NULL	NULL	0	NULL	six horses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In six horses , tendon lesions were created surgically in the Superficial Digital Flexor Tendons ( SDFT ) of both front limbs , one of which was treated with PRP and the other with saline .
	manualset3
103252	2	400456	5	NULL	NULL	0	NULL	tendon lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In six horses , tendon lesions were created surgically in the Superficial Digital Flexor Tendons ( SDFT ) of both front limbs , one of which was treated with PRP and the other with saline .
	manualset3
103253	3	400456	5	NULL	NULL	NULL	NULL	Superficial Digital Flexor Tendons ( SDFT )	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In six horses , tendon lesions were created surgically in the Superficial Digital Flexor Tendons ( SDFT ) of both front limbs , one of which was treated with PRP and the other with saline .
	manualset3
103254	4	400456	5	NULL	NULL	0	NULL	front limbs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In six horses , tendon lesions were created surgically in the Superficial Digital Flexor Tendons ( SDFT ) of both front limbs , one of which was treated with PRP and the other with saline .
	manualset3
103255	5	400456	5	NULL	NULL	0	NULL	PRP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In six horses , tendon lesions were created surgically in the Superficial Digital Flexor Tendons ( SDFT ) of both front limbs , one of which was treated with PRP and the other with saline .
	manualset3
103256	6	400456	5	NULL	NULL	0	NULL	saline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In six horses , tendon lesions were created surgically in the Superficial Digital Flexor Tendons ( SDFT ) of both front limbs , one of which was treated with PRP and the other with saline .
	manualset3
103257	1	400457	5	NULL	NULL	0	NULL	six patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In six patients the bony fragment was located in an unimproved medial position compared to the preoperative X-ray .
	manualset3
103258	2	400457	5	NULL	NULL	NULL	NULL	bony fragment	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In six patients the bony fragment was located in an unimproved medial position compared to the preoperative X-ray .
	manualset3
103259	3	400457	5	NULL	NULL	0	NULL	unimproved medial position	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In six patients the bony fragment was located in an unimproved medial position compared to the preoperative X-ray .
	manualset3
103260	4	400457	5	NULL	NULL	0	NULL	preoperative X-ray	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In six patients the bony fragment was located in an unimproved medial position compared to the preoperative X-ray .
	manualset3
103261	1	400458	5	NULL	NULL	0	NULL	 small islets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In small islets , - cells had abundant insulin content but limited amount of Golgi proinsulin .
	manualset3
103262	2	400458	5	NULL	NULL	0	NULL	 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In small islets , - cells had abundant insulin content but limited amount of Golgi proinsulin .
	manualset3
103263	3	400458	5	NULL	NULL	0	NULL	abundant insulin content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In small islets , - cells had abundant insulin content but limited amount of Golgi proinsulin .
	manualset3
103264	4	400458	5	NULL	NULL	0	NULL	limited amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In small islets , - cells had abundant insulin content but limited amount of Golgi proinsulin .
	manualset3
103265	5	400458	5	NULL	NULL	0	NULL	Golgi proinsulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In small islets , - cells had abundant insulin content but limited amount of Golgi proinsulin .
	manualset3
103266	1	400459	5	NULL	NULL	0	NULL	contribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	- The contribution of neoplasms to total mortality continues to increase .
	manualset3
103267	2	400459	5	NULL	NULL	0	NULL	neoplasms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	- The contribution of neoplasms to total mortality continues to increase .
	manualset3
103268	3	400459	5	NULL	NULL	NULL	NULL	total mortality	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	- The contribution of neoplasms to total mortality continues to increase .
	manualset3
103269	1	400460	5	NULL	NULL	0	NULL	soils	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In soils amended with CaCO ( 3 ) , S. marcescens did not die out , but the inhibition of A. niger by S. marcescens or Agrobacterium radiobacter was eliminated or reduced by the addition of glucose , but not of NH ( 4 ) NO ( 3 ) , and was influenced by the clay mineralogy and pH of the soils .
	manualset3
103270	2	400460	5	NULL	NULL	0	NULL	CaCO ( 3 )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In soils amended with CaCO ( 3 ) , S. marcescens did not die out , but the inhibition of A. niger by S. marcescens or Agrobacterium radiobacter was eliminated or reduced by the addition of glucose , but not of NH ( 4 ) NO ( 3 ) , and was influenced by the clay mineralogy and pH of the soils .
	manualset3
103271	3	400460	5	NULL	NULL	0	NULL	S. marcescens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In soils amended with CaCO ( 3 ) , S. marcescens did not die out , but the inhibition of A. niger by S. marcescens or Agrobacterium radiobacter was eliminated or reduced by the addition of glucose , but not of NH ( 4 ) NO ( 3 ) , and was influenced by the clay mineralogy and pH of the soils .
	manualset3
103272	4	400460	5	NULL	NULL	0	NULL	inhibition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In soils amended with CaCO ( 3 ) , S. marcescens did not die out , but the inhibition of A. niger by S. marcescens or Agrobacterium radiobacter was eliminated or reduced by the addition of glucose , but not of NH ( 4 ) NO ( 3 ) , and was influenced by the clay mineralogy and pH of the soils .
	manualset3
103273	5	400460	5	NULL	NULL	0	NULL	A. niger	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In soils amended with CaCO ( 3 ) , S. marcescens did not die out , but the inhibition of A. niger by S. marcescens or Agrobacterium radiobacter was eliminated or reduced by the addition of glucose , but not of NH ( 4 ) NO ( 3 ) , and was influenced by the clay mineralogy and pH of the soils .
	manualset3
103274	6	400460	5	NULL	NULL	0	NULL	S. marcescens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In soils amended with CaCO ( 3 ) , S. marcescens did not die out , but the inhibition of A. niger by S. marcescens or Agrobacterium radiobacter was eliminated or reduced by the addition of glucose , but not of NH ( 4 ) NO ( 3 ) , and was influenced by the clay mineralogy and pH of the soils .
	manualset3
103275	7	400460	5	NULL	NULL	0	NULL	Agrobacterium radiobacter	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In soils amended with CaCO ( 3 ) , S. marcescens did not die out , but the inhibition of A. niger by S. marcescens or Agrobacterium radiobacter was eliminated or reduced by the addition of glucose , but not of NH ( 4 ) NO ( 3 ) , and was influenced by the clay mineralogy and pH of the soils .
	manualset3
103276	8	400460	5	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In soils amended with CaCO ( 3 ) , S. marcescens did not die out , but the inhibition of A. niger by S. marcescens or Agrobacterium radiobacter was eliminated or reduced by the addition of glucose , but not of NH ( 4 ) NO ( 3 ) , and was influenced by the clay mineralogy and pH of the soils .
	manualset3
103277	9	400460	5	NULL	NULL	0	NULL	glucose 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In soils amended with CaCO ( 3 ) , S. marcescens did not die out , but the inhibition of A. niger by S. marcescens or Agrobacterium radiobacter was eliminated or reduced by the addition of glucose , but not of NH ( 4 ) NO ( 3 ) , and was influenced by the clay mineralogy and pH of the soils .
	manualset3
103278	10	400460	5	NULL	NULL	0	NULL	NH ( 4 ) NO ( 3 )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In soils amended with CaCO ( 3 ) , S. marcescens did not die out , but the inhibition of A. niger by S. marcescens or Agrobacterium radiobacter was eliminated or reduced by the addition of glucose , but not of NH ( 4 ) NO ( 3 ) , and was influenced by the clay mineralogy and pH of the soils .
	manualset3
103279	11	400460	5	NULL	NULL	0	NULL	clay mineralogy	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In soils amended with CaCO ( 3 ) , S. marcescens did not die out , but the inhibition of A. niger by S. marcescens or Agrobacterium radiobacter was eliminated or reduced by the addition of glucose , but not of NH ( 4 ) NO ( 3 ) , and was influenced by the clay mineralogy and pH of the soils .
	manualset3
103280	12	400460	5	NULL	NULL	0	NULL	pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In soils amended with CaCO ( 3 ) , S. marcescens did not die out , but the inhibition of A. niger by S. marcescens or Agrobacterium radiobacter was eliminated or reduced by the addition of glucose , but not of NH ( 4 ) NO ( 3 ) , and was influenced by the clay mineralogy and pH of the soils .
	manualset3
103281	13	400460	5	NULL	NULL	0	NULL	soils	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In soils amended with CaCO ( 3 ) , S. marcescens did not die out , but the inhibition of A. niger by S. marcescens or Agrobacterium radiobacter was eliminated or reduced by the addition of glucose , but not of NH ( 4 ) NO ( 3 ) , and was influenced by the clay mineralogy and pH of the soils .
	manualset3
103282	1	400461	5	NULL	NULL	0	NULL	soils	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In soils exposed to high levels ( 10 , 000 ppm ) of MeBr , methane oxidation was completely inhibited .
	manualset3
103283	2	400461	5	NULL	NULL	0	NULL	 high levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In soils exposed to high levels ( 10 , 000 ppm ) of MeBr , methane oxidation was completely inhibited .
	manualset3
103284	3	400461	5	NULL	NULL	0	NULL	10 , 000 ppm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In soils exposed to high levels ( 10 , 000 ppm ) of MeBr , methane oxidation was completely inhibited .
	manualset3
103285	4	400461	5	NULL	NULL	0	NULL	MeBr	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In soils exposed to high levels ( 10 , 000 ppm ) of MeBr , methane oxidation was completely inhibited .
	manualset3
103286	5	400461	5	NULL	NULL	0	NULL	methane oxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In soils exposed to high levels ( 10 , 000 ppm ) of MeBr , methane oxidation was completely inhibited .
	manualset3
103287	1	400462	5	NULL	NULL	0	NULL	cases	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In some cases , the appearance of lethal mutations was accompanied by the formation of inversions in the Xz chromosome .
	manualset3
103288	2	400462	5	NULL	NULL	0	NULL	appearance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In some cases , the appearance of lethal mutations was accompanied by the formation of inversions in the Xz chromosome .
	manualset3
103289	3	400462	5	NULL	NULL	0	NULL	lethal mutations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In some cases , the appearance of lethal mutations was accompanied by the formation of inversions in the Xz chromosome .
	manualset3
103290	4	400462	5	NULL	NULL	0	NULL	formation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In some cases , the appearance of lethal mutations was accompanied by the formation of inversions in the Xz chromosome .
	manualset3
103291	5	400462	5	NULL	NULL	0	NULL	inversions 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In some cases , the appearance of lethal mutations was accompanied by the formation of inversions in the Xz chromosome .
	manualset3
103292	6	400462	5	NULL	NULL	NULL	NULL	Xz chromosome 	Chromosome												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In some cases , the appearance of lethal mutations was accompanied by the formation of inversions in the Xz chromosome .
	manualset3
103293	1	400463	5	NULL	NULL	0	NULL	cases 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In some cases , the procedure was repeated using a continuous , broadband noise masker ( 20-50 dB/Hz ) .
	manualset3
103294	2	400463	5	NULL	NULL	0	NULL	procedure 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In some cases , the procedure was repeated using a continuous , broadband noise masker ( 20-50 dB/Hz ) .
	manualset3
103295	3	400463	5	NULL	NULL	0	NULL	continuous , broadband noise masker	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In some cases , the procedure was repeated using a continuous , broadband noise masker ( 20-50 dB/Hz ) .
	manualset3
103296	4	400463	5	NULL	NULL	0	NULL	20-50 dB/Hz	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In some cases , the procedure was repeated using a continuous , broadband noise masker ( 20-50 dB/Hz ) .
	manualset3
103297	1	400464	5	NULL	NULL	0	NULL	temporary internal portocaval shunt	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In some instances , a temporary internal portocaval shunt is constructed to relieve hemodynamic instability .
	manualset3
103298	2	400464	5	NULL	NULL	0	NULL	hemodynamic instability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In some instances , a temporary internal portocaval shunt is constructed to relieve hemodynamic instability .
	manualset3
103299	1	400465	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In some patients , however , I-131 MIBG may fail to localize pheochromocytoma .
	manualset3
103300	2	400465	5	NULL	NULL	0	NULL	I-131 MIBG	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In some patients , however , I-131 MIBG may fail to localize pheochromocytoma .
	manualset3
103301	3	400465	5	NULL	NULL	0	NULL	pheochromocytoma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In some patients , however , I-131 MIBG may fail to localize pheochromocytoma .
	manualset3
103302	1	400466	5	NULL	NULL	0	NULL	rhizobia 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In some rhizobia , mutation of genes involved in cytochrome c assembly does not strongly affect growth , presumably because the bacteria utilize the cytochrome c-independent quinol oxidases .
	manualset3
103303	2	400466	5	NULL	NULL	0	NULL	mutation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In some rhizobia , mutation of genes involved in cytochrome c assembly does not strongly affect growth , presumably because the bacteria utilize the cytochrome c-independent quinol oxidases .
	manualset3
103304	3	400466	5	NULL	NULL	0	NULL	genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In some rhizobia , mutation of genes involved in cytochrome c assembly does not strongly affect growth , presumably because the bacteria utilize the cytochrome c-independent quinol oxidases .
	manualset3
103305	4	400466	5	NULL	NULL	0	NULL	cytochrome c assembly	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In some rhizobia , mutation of genes involved in cytochrome c assembly does not strongly affect growth , presumably because the bacteria utilize the cytochrome c-independent quinol oxidases .
	manualset3
103306	5	400466	5	NULL	NULL	0	NULL	growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In some rhizobia , mutation of genes involved in cytochrome c assembly does not strongly affect growth , presumably because the bacteria utilize the cytochrome c-independent quinol oxidases .
	manualset3
103307	6	400466	5	NULL	NULL	0	NULL	bacteria 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In some rhizobia , mutation of genes involved in cytochrome c assembly does not strongly affect growth , presumably because the bacteria utilize the cytochrome c-independent quinol oxidases .
	manualset3
103308	7	400466	5	NULL	NULL	0	NULL	cytochrome c-independent quinol oxidases	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In some rhizobia , mutation of genes involved in cytochrome c assembly does not strongly affect growth , presumably because the bacteria utilize the cytochrome c-independent quinol oxidases .
	manualset3
103309	1	400467	5	NULL	NULL	0	NULL	biologicals	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	- These biologicals include both soluble immune-receptor proteins and monoclonal antibodies that are aimed at immune mediators , receptors or cells .
	manualset3
103310	2	400467	5	NULL	NULL	NULL	NULL	soluble immune-receptor proteins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	- These biologicals include both soluble immune-receptor proteins and monoclonal antibodies that are aimed at immune mediators , receptors or cells .
	manualset3
103311	3	400467	5	NULL	NULL	0	NULL	monoclonal antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	- These biologicals include both soluble immune-receptor proteins and monoclonal antibodies that are aimed at immune mediators , receptors or cells .
	manualset3
103312	4	400467	5	NULL	NULL	NULL	NULL	immune mediators	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	- These biologicals include both soluble immune-receptor proteins and monoclonal antibodies that are aimed at immune mediators , receptors or cells .
	manualset3
103313	5	400467	5	NULL	NULL	0	NULL	receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	- These biologicals include both soluble immune-receptor proteins and monoclonal antibodies that are aimed at immune mediators , receptors or cells .
	manualset3
103314	6	400467	5	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	- These biologicals include both soluble immune-receptor proteins and monoclonal antibodies that are aimed at immune mediators , receptors or cells .
	manualset3
103315	1	400468	5	NULL	NULL	0	NULL	state of preparation 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In some state of preparation the size of potential evoked by a constant number of stimuli was nearly constant , being independent from stimulus frequencies , that is , pattern insensitive .
	manualset3
103316	2	400468	5	NULL	NULL	0	NULL	size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In some state of preparation the size of potential evoked by a constant number of stimuli was nearly constant , being independent from stimulus frequencies , that is , pattern insensitive .
	manualset3
103317	3	400468	5	NULL	NULL	0	NULL	potential	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In some state of preparation the size of potential evoked by a constant number of stimuli was nearly constant , being independent from stimulus frequencies , that is , pattern insensitive .
	manualset3
103318	4	400468	5	NULL	NULL	0	NULL	constant number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In some state of preparation the size of potential evoked by a constant number of stimuli was nearly constant , being independent from stimulus frequencies , that is , pattern insensitive .
	manualset3
103319	5	400468	5	NULL	NULL	0	NULL	stimuli 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In some state of preparation the size of potential evoked by a constant number of stimuli was nearly constant , being independent from stimulus frequencies , that is , pattern insensitive .
	manualset3
103321	6	400468	5	NULL	NULL	NULL	NULL	stimulus frequencies	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In some state of preparation the size of potential evoked by a constant number of stimuli was nearly constant , being independent from stimulus frequencies , that is , pattern insensitive .
	manualset3
103322	1	400469	5	NULL	NULL	0	NULL	tests	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In some tests , chlorpromazine served as a reference drug .
	manualset3
103323	2	400469	5	NULL	NULL	0	NULL	chlorpromazine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In some tests , chlorpromazine served as a reference drug .
	manualset3
103324	3	400469	5	NULL	NULL	0	NULL	reference drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In some tests , chlorpromazine served as a reference drug .
	manualset3
103325	1	400470	5	NULL	NULL	0	NULL	limited number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of a limited number of studies , object recognition does not seem dramatically altered by weightlessness and astronauts can adapt to this novel environment .
	manualset3
103326	2	400470	5	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of a limited number of studies , object recognition does not seem dramatically altered by weightlessness and astronauts can adapt to this novel environment .
	manualset3
103327	3	400470	5	NULL	NULL	0	NULL	object recognition	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of a limited number of studies , object recognition does not seem dramatically altered by weightlessness and astronauts can adapt to this novel environment .
	manualset3
103328	4	400470	5	NULL	NULL	0	NULL	astronauts 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of a limited number of studies , object recognition does not seem dramatically altered by weightlessness and astronauts can adapt to this novel environment .
	manualset3
103329	5	400470	5	NULL	NULL	0	NULL	novel environment	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of a limited number of studies , object recognition does not seem dramatically altered by weightlessness and astronauts can adapt to this novel environment .
	manualset3
103330	1	400471	5	NULL	NULL	0	NULL	significantly higher inhibitor levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of significantly higher inhibitor levels in the neoplastic tissues , u-PA was found to be increased as well , both in antigen level and in activity .
	manualset3
103331	2	400471	5	NULL	NULL	0	NULL	neoplastic tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of significantly higher inhibitor levels in the neoplastic tissues , u-PA was found to be increased as well , both in antigen level and in activity .
	manualset3
103332	3	400471	5	NULL	NULL	0	NULL	u-PA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of significantly higher inhibitor levels in the neoplastic tissues , u-PA was found to be increased as well , both in antigen level and in activity .
	manualset3
103333	4	400471	5	NULL	NULL	0	NULL	antigen level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of significantly higher inhibitor levels in the neoplastic tissues , u-PA was found to be increased as well , both in antigen level and in activity .
	manualset3
103334	5	400471	5	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of significantly higher inhibitor levels in the neoplastic tissues , u-PA was found to be increased as well , both in antigen level and in activity .
	manualset3
103335	1	400472	5	NULL	NULL	0	NULL	standardization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of standardization of surgical procedures in the treatment of gastric carcinomas including increased resection rates as well as decreased postoperative mortality long-term survival rates are poor .
	manualset3
103336	2	400472	5	NULL	NULL	0	NULL	surgical procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of standardization of surgical procedures in the treatment of gastric carcinomas including increased resection rates as well as decreased postoperative mortality long-term survival rates are poor .
	manualset3
103337	3	400472	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of standardization of surgical procedures in the treatment of gastric carcinomas including increased resection rates as well as decreased postoperative mortality long-term survival rates are poor .
	manualset3
103338	4	400472	5	NULL	NULL	0	NULL	gastric carcinomas 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of standardization of surgical procedures in the treatment of gastric carcinomas including increased resection rates as well as decreased postoperative mortality long-term survival rates are poor .
	manualset3
103339	5	400472	5	NULL	NULL	0	NULL	increased resection rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of standardization of surgical procedures in the treatment of gastric carcinomas including increased resection rates as well as decreased postoperative mortality long-term survival rates are poor .
	manualset3
103340	6	400472	5	NULL	NULL	0	NULL	decreased postoperative mortality	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of standardization of surgical procedures in the treatment of gastric carcinomas including increased resection rates as well as decreased postoperative mortality long-term survival rates are poor .
	manualset3
103341	7	400472	5	NULL	NULL	0	NULL	long-term survival rates 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of standardization of surgical procedures in the treatment of gastric carcinomas including increased resection rates as well as decreased postoperative mortality long-term survival rates are poor .
	manualset3
103342	1	400473	5	NULL	NULL	0	NULL	 2-phenyl flavonoids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of the 2-phenyl flavonoids , some tested compounds did not show any insect antifeedant activity against the common cutworm , although these inactive flavonoids were deficient in the 6-substituent group on the A-ring of the flavonoid .
	manualset3
103343	2	400473	5	NULL	NULL	0	NULL	tested compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of the 2-phenyl flavonoids , some tested compounds did not show any insect antifeedant activity against the common cutworm , although these inactive flavonoids were deficient in the 6-substituent group on the A-ring of the flavonoid .
	manualset3
103344	3	400473	5	NULL	NULL	0	NULL	insect antifeedant activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of the 2-phenyl flavonoids , some tested compounds did not show any insect antifeedant activity against the common cutworm , although these inactive flavonoids were deficient in the 6-substituent group on the A-ring of the flavonoid .
	manualset3
103345	4	400473	5	NULL	NULL	0	NULL	common cutworm	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of the 2-phenyl flavonoids , some tested compounds did not show any insect antifeedant activity against the common cutworm , although these inactive flavonoids were deficient in the 6-substituent group on the A-ring of the flavonoid .
	manualset3
103346	5	400473	5	NULL	NULL	0	NULL	inactive flavonoids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of the 2-phenyl flavonoids , some tested compounds did not show any insect antifeedant activity against the common cutworm , although these inactive flavonoids were deficient in the 6-substituent group on the A-ring of the flavonoid .
	manualset3
103347	6	400473	5	NULL	NULL	0	NULL	6-substituent group	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of the 2-phenyl flavonoids , some tested compounds did not show any insect antifeedant activity against the common cutworm , although these inactive flavonoids were deficient in the 6-substituent group on the A-ring of the flavonoid .
	manualset3
103348	7	400473	5	NULL	NULL	0	NULL	A-ring of the flavonoid	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of the 2-phenyl flavonoids , some tested compounds did not show any insect antifeedant activity against the common cutworm , although these inactive flavonoids were deficient in the 6-substituent group on the A-ring of the flavonoid .
	manualset3
103349	1	400474	5	NULL	NULL	0	NULL	different pressure load	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of the different pressure load of the right ventricle after hypoxia in treated and control rats , there was no difference in parameters indicative of the degree of right ventricular hypertrophy between these two groups of hypoxic rats .
	manualset3
103350	2	400474	5	NULL	NULL	0	NULL	right ventricle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of the different pressure load of the right ventricle after hypoxia in treated and control rats , there was no difference in parameters indicative of the degree of right ventricular hypertrophy between these two groups of hypoxic rats .
	manualset3
103351	3	400474	5	NULL	NULL	0	NULL	hypoxia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of the different pressure load of the right ventricle after hypoxia in treated and control rats , there was no difference in parameters indicative of the degree of right ventricular hypertrophy between these two groups of hypoxic rats .
	manualset3
103352	4	400474	5	NULL	NULL	0	NULL	control rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of the different pressure load of the right ventricle after hypoxia in treated and control rats , there was no difference in parameters indicative of the degree of right ventricular hypertrophy between these two groups of hypoxic rats .
	manualset3
103353	5	400474	5	NULL	NULL	0	NULL	difference 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of the different pressure load of the right ventricle after hypoxia in treated and control rats , there was no difference in parameters indicative of the degree of right ventricular hypertrophy between these two groups of hypoxic rats .
	manualset3
103354	6	400474	5	NULL	NULL	0	NULL	parameters 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of the different pressure load of the right ventricle after hypoxia in treated and control rats , there was no difference in parameters indicative of the degree of right ventricular hypertrophy between these two groups of hypoxic rats .
	manualset3
103355	7	400474	5	NULL	NULL	0	NULL	degree 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of the different pressure load of the right ventricle after hypoxia in treated and control rats , there was no difference in parameters indicative of the degree of right ventricular hypertrophy between these two groups of hypoxic rats .
	manualset3
103356	8	400474	5	NULL	NULL	0	NULL	right ventricular hypertrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of the different pressure load of the right ventricle after hypoxia in treated and control rats , there was no difference in parameters indicative of the degree of right ventricular hypertrophy between these two groups of hypoxic rats .
	manualset3
103357	9	400474	5	NULL	NULL	0	NULL	two groups	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of the different pressure load of the right ventricle after hypoxia in treated and control rats , there was no difference in parameters indicative of the degree of right ventricular hypertrophy between these two groups of hypoxic rats .
	manualset3
103358	10	400474	5	NULL	NULL	0	NULL	hypoxic rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of the different pressure load of the right ventricle after hypoxia in treated and control rats , there was no difference in parameters indicative of the degree of right ventricular hypertrophy between these two groups of hypoxic rats .
	manualset3
103360	1	400475	5	NULL	NULL	0	NULL	arrestins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	- arrestins therefore seem to regulate an endosome to Golgi pathway used by multiple cargo proteins .
	manualset3
103361	2	400475	5	NULL	NULL	0	NULL	regulate 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	- arrestins therefore seem to regulate an endosome to Golgi pathway used by multiple cargo proteins .
	manualset3
103362	3	400475	5	NULL	NULL	0	NULL	endosome 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	- arrestins therefore seem to regulate an endosome to Golgi pathway used by multiple cargo proteins .
	manualset3
103363	4	400475	5	NULL	NULL	0	NULL	Golgi pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	- arrestins therefore seem to regulate an endosome to Golgi pathway used by multiple cargo proteins .
	manualset3
103364	5	400475	5	NULL	NULL	0	NULL	multiple cargo proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	- arrestins therefore seem to regulate an endosome to Golgi pathway used by multiple cargo proteins .
	manualset3
103365	1	400476	5	NULL	NULL	0	NULL	relatively small differences	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of the relatively small differences in the chemical structures of the compounds studied , large differences were observed in their binding behaviors to plasmatic proteins .
	manualset3
103366	2	400476	5	NULL	NULL	0	NULL	chemical structures	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of the relatively small differences in the chemical structures of the compounds studied , large differences were observed in their binding behaviors to plasmatic proteins .
	manualset3
103367	3	400476	5	NULL	NULL	0	NULL	compounds 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of the relatively small differences in the chemical structures of the compounds studied , large differences were observed in their binding behaviors to plasmatic proteins .
	manualset3
103368	4	400476	5	NULL	NULL	0	NULL	large differences	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of the relatively small differences in the chemical structures of the compounds studied , large differences were observed in their binding behaviors to plasmatic proteins .
	manualset3
103369	5	400476	5	NULL	NULL	0	NULL	binding behaviors	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of the relatively small differences in the chemical structures of the compounds studied , large differences were observed in their binding behaviors to plasmatic proteins .
	manualset3
103370	6	400476	5	NULL	NULL	0	NULL	plasmatic proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of the relatively small differences in the chemical structures of the compounds studied , large differences were observed in their binding behaviors to plasmatic proteins .
	manualset3
103371	1	400477	5	NULL	NULL	0	NULL	pathological changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of these pathological changes , the original framework of the alveolar wall is preserved in many areas .
	manualset3
103372	2	400477	5	NULL	NULL	0	NULL	original framework	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of these pathological changes , the original framework of the alveolar wall is preserved in many areas .
	manualset3
103373	3	400477	5	NULL	NULL	0	NULL	alveolar wall	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of these pathological changes , the original framework of the alveolar wall is preserved in many areas .
	manualset3
103374	4	400477	5	NULL	NULL	0	NULL	areas	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of these pathological changes , the original framework of the alveolar wall is preserved in many areas .
	manualset3
103375	1	400478	5	NULL	NULL	0	NULL	vigorous antibiotic therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of vigorous antibiotic therapy fever and positive blood cultures persisted .
	manualset3
103376	2	400478	5	NULL	NULL	0	NULL	fever	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of vigorous antibiotic therapy fever and positive blood cultures persisted .
	manualset3
103377	3	400478	5	NULL	NULL	0	NULL	positive blood cultures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In spite of vigorous antibiotic therapy fever and positive blood cultures persisted .
	manualset3
103378	1	400479	5	NULL	NULL	0	NULL	spleen cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In spleen cells , calcium chelation with EGTA triggered apoptosis .
	manualset3
103379	2	400479	5	NULL	NULL	0	NULL	calcium chelation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In spleen cells , calcium chelation with EGTA triggered apoptosis .
	manualset3
103380	3	400479	5	NULL	NULL	0	NULL	EGTA 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In spleen cells , calcium chelation with EGTA triggered apoptosis .
	manualset3
103381	4	400479	5	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In spleen cells , calcium chelation with EGTA triggered apoptosis .
	manualset3
103382	1	400480	5	NULL	NULL	NULL	NULL	stage I pts	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In stage I pts ER distribution showed lower values in pts with relapse , as compared to the group without relapse ( 0-115 vs. 0-464 ) , and a tendency for relapse occurrence below the ER levels of 33 fmol/mg .
	manualset3
103557	2	400480	5	NULL	NULL	0	NULL	ER distribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In stage I pts ER distribution showed lower values in pts with relapse , as compared to the group without relapse ( 0-115 vs. 0-464 ) , and a tendency for relapse occurrence below the ER levels of 33 fmol/mg .
	manualset3
103558	3	400480	5	NULL	NULL	0	NULL	lower values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In stage I pts ER distribution showed lower values in pts with relapse , as compared to the group without relapse ( 0-115 vs. 0-464 ) , and a tendency for relapse occurrence below the ER levels of 33 fmol/mg .
	manualset3
103559	4	400480	5	NULL	NULL	0	NULL	pts	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In stage I pts ER distribution showed lower values in pts with relapse , as compared to the group without relapse ( 0-115 vs. 0-464 ) , and a tendency for relapse occurrence below the ER levels of 33 fmol/mg .
	manualset3
103560	5	400480	5	NULL	NULL	0	NULL	relapse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In stage I pts ER distribution showed lower values in pts with relapse , as compared to the group without relapse ( 0-115 vs. 0-464 ) , and a tendency for relapse occurrence below the ER levels of 33 fmol/mg .
	manualset3
103561	6	400480	5	NULL	NULL	0	NULL	group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In stage I pts ER distribution showed lower values in pts with relapse , as compared to the group without relapse ( 0-115 vs. 0-464 ) , and a tendency for relapse occurrence below the ER levels of 33 fmol/mg .
	manualset3
103562	7	400480	5	NULL	NULL	0	NULL	relapse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In stage I pts ER distribution showed lower values in pts with relapse , as compared to the group without relapse ( 0-115 vs. 0-464 ) , and a tendency for relapse occurrence below the ER levels of 33 fmol/mg .
	manualset3
103563	8	400480	5	NULL	NULL	0	NULL	0-115 vs. 0-464	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In stage I pts ER distribution showed lower values in pts with relapse , as compared to the group without relapse ( 0-115 vs. 0-464 ) , and a tendency for relapse occurrence below the ER levels of 33 fmol/mg .
	manualset3
103564	9	400480	5	NULL	NULL	NULL	NULL	relapse occurence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In stage I pts ER distribution showed lower values in pts with relapse , as compared to the group without relapse ( 0-115 vs. 0-464 ) , and a tendency for relapse occurrence below the ER levels of 33 fmol/mg .
	manualset3
103565	10	400480	5	NULL	NULL	0	NULL	ER levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In stage I pts ER distribution showed lower values in pts with relapse , as compared to the group without relapse ( 0-115 vs. 0-464 ) , and a tendency for relapse occurrence below the ER levels of 33 fmol/mg .
	manualset3
103566	11	400480	5	NULL	NULL	0	NULL	33 fmol/mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In stage I pts ER distribution showed lower values in pts with relapse , as compared to the group without relapse ( 0-115 vs. 0-464 ) , and a tendency for relapse occurrence below the ER levels of 33 fmol/mg .
	manualset3
103567	1	400481	5	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In studies of raloxifene as treatment for osteoporosis , when viewed as a secondary endpoint there was a significant reduction in risk of new onset breast cancer .
	manualset3
103568	2	400481	5	NULL	NULL	0	NULL	raloxifene	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In studies of raloxifene as treatment for osteoporosis , when viewed as a secondary endpoint there was a significant reduction in risk of new onset breast cancer .
	manualset3
103569	3	400481	5	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In studies of raloxifene as treatment for osteoporosis , when viewed as a secondary endpoint there was a significant reduction in risk of new onset breast cancer .
	manualset3
103570	4	400481	5	NULL	NULL	0	NULL	osteoporosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In studies of raloxifene as treatment for osteoporosis , when viewed as a secondary endpoint there was a significant reduction in risk of new onset breast cancer .
	manualset3
103571	5	400481	5	NULL	NULL	0	NULL	secondary endpoint 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In studies of raloxifene as treatment for osteoporosis , when viewed as a secondary endpoint there was a significant reduction in risk of new onset breast cancer .
	manualset3
103572	6	400481	5	NULL	NULL	0	NULL	risk	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In studies of raloxifene as treatment for osteoporosis , when viewed as a secondary endpoint there was a significant reduction in risk of new onset breast cancer .
	manualset3
103573	7	400481	5	NULL	NULL	0	NULL	breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In studies of raloxifene as treatment for osteoporosis , when viewed as a secondary endpoint there was a significant reduction in risk of new onset breast cancer .
	manualset3
103574	1	400482	5	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In studies on the formation and persistence of the 1 , 8-NONO2 adduct in RTEC maximum binding was observed at 1 h. Fifteen hours later the RAL value was less than 15 % of this maximum level .
	manualset3
103575	2	400482	5	NULL	NULL	0	NULL	formation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In studies on the formation and persistence of the 1 , 8-NONO2 adduct in RTEC maximum binding was observed at 1 h. Fifteen hours later the RAL value was less than 15 % of this maximum level .
	manualset3
103576	3	400482	5	NULL	NULL	0	NULL	persistence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In studies on the formation and persistence of the 1 , 8-NONO2 adduct in RTEC maximum binding was observed at 1 h. Fifteen hours later the RAL value was less than 15 % of this maximum level .
	manualset3
103577	4	400482	5	NULL	NULL	NULL	NULL	1 , 8-NONO2 adduct	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In studies on the formation and persistence of the 1 , 8-NONO2 adduct in RTEC maximum binding was observed at 1 h. Fifteen hours later the RAL value was less than 15 % of this maximum level .
	manualset3
103578	5	400482	5	NULL	NULL	0	NULL	RTEC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In studies on the formation and persistence of the 1 , 8-NONO2 adduct in RTEC maximum binding was observed at 1 h. Fifteen hours later the RAL value was less than 15 % of this maximum level .
	manualset3
103579	6	400482	5	NULL	NULL	0	NULL	1 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In studies on the formation and persistence of the 1 , 8-NONO2 adduct in RTEC maximum binding was observed at 1 h. Fifteen hours later the RAL value was less than 15 % of this maximum level .
	manualset3
103580	7	400482	5	NULL	NULL	0	NULL	Fifteen hours	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In studies on the formation and persistence of the 1 , 8-NONO2 adduct in RTEC maximum binding was observed at 1 h. Fifteen hours later the RAL value was less than 15 % of this maximum level .
	manualset3
103581	8	400482	5	NULL	NULL	0	NULL	RAL value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In studies on the formation and persistence of the 1 , 8-NONO2 adduct in RTEC maximum binding was observed at 1 h. Fifteen hours later the RAL value was less than 15 % of this maximum level .
	manualset3
103582	9	400482	5	NULL	NULL	0	NULL	15 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In studies on the formation and persistence of the 1 , 8-NONO2 adduct in RTEC maximum binding was observed at 1 h. Fifteen hours later the RAL value was less than 15 % of this maximum level .
	manualset3
103583	10	400482	5	NULL	NULL	0	NULL	maximum level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In studies on the formation and persistence of the 1 , 8-NONO2 adduct in RTEC maximum binding was observed at 1 h. Fifteen hours later the RAL value was less than 15 % of this maximum level .
	manualset3
103584	1	400483	5	NULL	NULL	0	NULL	Application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Application of the automatic Edman procedure to establishing the primary structure of swine pepsinogen and its fragments ) .
	manualset3
103585	2	400483	5	NULL	NULL	0	NULL	automatic Edman procedure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Application of the automatic Edman procedure to establishing the primary structure of swine pepsinogen and its fragments ) .
	manualset3
103586	3	400483	5	NULL	NULL	0	NULL	primary structure 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Application of the automatic Edman procedure to establishing the primary structure of swine pepsinogen and its fragments ) .
	manualset3
103587	4	400483	5	NULL	NULL	0	NULL	swine pepsinogen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Application of the automatic Edman procedure to establishing the primary structure of swine pepsinogen and its fragments ) .
	manualset3
103588	5	400483	5	NULL	NULL	0	NULL	swine pepsinogen fragments	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Application of the automatic Edman procedure to establishing the primary structure of swine pepsinogen and its fragments ) .
	manualset3
103589	1	400484	5	NULL	NULL	0	NULL	catenin	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	- catenin is a molecular switch that regulates transition of cell-cell adhesion to fusion .
	manualset3
103590	2	400484	5	NULL	NULL	0	NULL	molecular switch	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	- catenin is a molecular switch that regulates transition of cell-cell adhesion to fusion .
	manualset3
103591	3	400484	5	NULL	NULL	0	NULL	transition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	- catenin is a molecular switch that regulates transition of cell-cell adhesion to fusion .
	manualset3
103592	4	400484	5	NULL	NULL	0	NULL	cell-cell adhesion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	- catenin is a molecular switch that regulates transition of cell-cell adhesion to fusion .
	manualset3
103593	5	400484	5	NULL	NULL	0	NULL	fusion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	- catenin is a molecular switch that regulates transition of cell-cell adhesion to fusion .
	manualset3
103594	1	400485	5	NULL	NULL	0	NULL	conditions	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In such conditions , LU 105 at 0.1 % , 0.01 % , and 0.001 % developed a dose dependent protection of gingival elastic fibers against enzymatic proteolysis due to human leukocyte elastase , and LU 105 at 0.1 % or 0.01 % was able to inhibit the elastolytic activity of leukocyte elastase itself .
	manualset3
103595	2	400485	5	NULL	NULL	0	NULL	LU 105	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In such conditions , LU 105 at 0.1 % , 0.01 % , and 0.001 % developed a dose dependent protection of gingival elastic fibers against enzymatic proteolysis due to human leukocyte elastase , and LU 105 at 0.1 % or 0.01 % was able to inhibit the elastolytic activity of leukocyte elastase itself .
	manualset3
103596	3	400485	5	NULL	NULL	0	NULL	0.1 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In such conditions , LU 105 at 0.1 % , 0.01 % , and 0.001 % developed a dose dependent protection of gingival elastic fibers against enzymatic proteolysis due to human leukocyte elastase , and LU 105 at 0.1 % or 0.01 % was able to inhibit the elastolytic activity of leukocyte elastase itself .
	manualset3
103597	4	400485	5	NULL	NULL	0	NULL	0.01 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In such conditions , LU 105 at 0.1 % , 0.01 % , and 0.001 % developed a dose dependent protection of gingival elastic fibers against enzymatic proteolysis due to human leukocyte elastase , and LU 105 at 0.1 % or 0.01 % was able to inhibit the elastolytic activity of leukocyte elastase itself .
	manualset3
103598	5	400485	5	NULL	NULL	0	NULL	0.001 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In such conditions , LU 105 at 0.1 % , 0.01 % , and 0.001 % developed a dose dependent protection of gingival elastic fibers against enzymatic proteolysis due to human leukocyte elastase , and LU 105 at 0.1 % or 0.01 % was able to inhibit the elastolytic activity of leukocyte elastase itself .
	manualset3
103599	6	400485	5	NULL	NULL	0	NULL	dose dependent protection	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In such conditions , LU 105 at 0.1 % , 0.01 % , and 0.001 % developed a dose dependent protection of gingival elastic fibers against enzymatic proteolysis due to human leukocyte elastase , and LU 105 at 0.1 % or 0.01 % was able to inhibit the elastolytic activity of leukocyte elastase itself .
	manualset3
103600	7	400485	5	NULL	NULL	0	NULL	gingival elastic fibers	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In such conditions , LU 105 at 0.1 % , 0.01 % , and 0.001 % developed a dose dependent protection of gingival elastic fibers against enzymatic proteolysis due to human leukocyte elastase , and LU 105 at 0.1 % or 0.01 % was able to inhibit the elastolytic activity of leukocyte elastase itself .
	manualset3
103601	8	400485	5	NULL	NULL	0	NULL	enzymatic proteolysis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In such conditions , LU 105 at 0.1 % , 0.01 % , and 0.001 % developed a dose dependent protection of gingival elastic fibers against enzymatic proteolysis due to human leukocyte elastase , and LU 105 at 0.1 % or 0.01 % was able to inhibit the elastolytic activity of leukocyte elastase itself .
	manualset3
103602	9	400485	5	NULL	NULL	0	NULL	human leukocyte elastase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In such conditions , LU 105 at 0.1 % , 0.01 % , and 0.001 % developed a dose dependent protection of gingival elastic fibers against enzymatic proteolysis due to human leukocyte elastase , and LU 105 at 0.1 % or 0.01 % was able to inhibit the elastolytic activity of leukocyte elastase itself .
	manualset3
103603	10	400485	5	NULL	NULL	0	NULL	LU 105	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In such conditions , LU 105 at 0.1 % , 0.01 % , and 0.001 % developed a dose dependent protection of gingival elastic fibers against enzymatic proteolysis due to human leukocyte elastase , and LU 105 at 0.1 % or 0.01 % was able to inhibit the elastolytic activity of leukocyte elastase itself .
	manualset3
103604	11	400485	5	NULL	NULL	0	NULL	0.1 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In such conditions , LU 105 at 0.1 % , 0.01 % , and 0.001 % developed a dose dependent protection of gingival elastic fibers against enzymatic proteolysis due to human leukocyte elastase , and LU 105 at 0.1 % or 0.01 % was able to inhibit the elastolytic activity of leukocyte elastase itself .
	manualset3
103605	12	400485	5	NULL	NULL	0	NULL	0.01 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In such conditions , LU 105 at 0.1 % , 0.01 % , and 0.001 % developed a dose dependent protection of gingival elastic fibers against enzymatic proteolysis due to human leukocyte elastase , and LU 105 at 0.1 % or 0.01 % was able to inhibit the elastolytic activity of leukocyte elastase itself .
	manualset3
103606	13	400485	5	NULL	NULL	0	NULL	elastolytic activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In such conditions , LU 105 at 0.1 % , 0.01 % , and 0.001 % developed a dose dependent protection of gingival elastic fibers against enzymatic proteolysis due to human leukocyte elastase , and LU 105 at 0.1 % or 0.01 % was able to inhibit the elastolytic activity of leukocyte elastase itself .
	manualset3
103607	14	400485	5	NULL	NULL	0	NULL	leukocyte elastase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In such conditions , LU 105 at 0.1 % , 0.01 % , and 0.001 % developed a dose dependent protection of gingival elastic fibers against enzymatic proteolysis due to human leukocyte elastase , and LU 105 at 0.1 % or 0.01 % was able to inhibit the elastolytic activity of leukocyte elastase itself .
	manualset3
103608	1	400486	5	NULL	NULL	0	NULL	images	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In such images , iris textures are almost invisible , making them unsuited for direct application of standard matching algorithms , which are used to calculate torsional eye movements .
	manualset3
103609	2	400486	5	NULL	NULL	0	NULL	iris textures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In such images , iris textures are almost invisible , making them unsuited for direct application of standard matching algorithms , which are used to calculate torsional eye movements .
	manualset3
103610	3	400486	5	NULL	NULL	0	NULL	direct application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In such images , iris textures are almost invisible , making them unsuited for direct application of standard matching algorithms , which are used to calculate torsional eye movements .
	manualset3
103611	4	400486	5	NULL	NULL	0	NULL	standard matching algorithms	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In such images , iris textures are almost invisible , making them unsuited for direct application of standard matching algorithms , which are used to calculate torsional eye movements .
	manualset3
103613	5	400486	5	NULL	NULL	NULL	NULL	torsional eye movements	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In such images , iris textures are almost invisible , making them unsuited for direct application of standard matching algorithms , which are used to calculate torsional eye movements .
	manualset3
103614	1	400487	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In such patients , a steep increase in mortality rates has been observed .
	manualset3
103615	2	400487	5	NULL	NULL	0	NULL	mortality rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In such patients , a steep increase in mortality rates has been observed .
	manualset3
107681	3	400487	5	NULL	NULL	0	NULL	steep increase	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In such patients , a steep increase in mortality rates has been observed .
	manualset3
103616	1	400488	5	NULL	NULL	0	NULL	plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In such plants neither PVY-NIa nor spacer transgene transcripts were detectable by specific quantitative real time reverse transcriptase PCR ( RT-qPCR ) assays of similar relative efficiencies developed for direct comparative analysis .
	manualset3
103617	2	400488	5	NULL	NULL	0	NULL	PVY-NIa	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In such plants neither PVY-NIa nor spacer transgene transcripts were detectable by specific quantitative real time reverse transcriptase PCR ( RT-qPCR ) assays of similar relative efficiencies developed for direct comparative analysis .
	manualset3
103618	3	400488	5	NULL	NULL	0	NULL	spacer transgene transcripts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In such plants neither PVY-NIa nor spacer transgene transcripts were detectable by specific quantitative real time reverse transcriptase PCR ( RT-qPCR ) assays of similar relative efficiencies developed for direct comparative analysis .
	manualset3
103619	4	400488	5	NULL	NULL	0	NULL	quantitative real time reverse transcriptase PCR ( RT-qPCR ) assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In such plants neither PVY-NIa nor spacer transgene transcripts were detectable by specific quantitative real time reverse transcriptase PCR ( RT-qPCR ) assays of similar relative efficiencies developed for direct comparative analysis .
	manualset3
103620	5	400488	5	NULL	NULL	0	NULL	relative efficiencies	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In such plants neither PVY-NIa nor spacer transgene transcripts were detectable by specific quantitative real time reverse transcriptase PCR ( RT-qPCR ) assays of similar relative efficiencies developed for direct comparative analysis .
	manualset3
103621	6	400488	5	NULL	NULL	0	NULL	direct comparative analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In such plants neither PVY-NIa nor spacer transgene transcripts were detectable by specific quantitative real time reverse transcriptase PCR ( RT-qPCR ) assays of similar relative efficiencies developed for direct comparative analysis .
	manualset3
103622	1	400489	5	NULL	NULL	0	NULL	system 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In such a system , spins are filtered not only by spin matching-mismatching between both electrodes as in normal spin-valve devices , but also by the orbital symmetry matching-mismatching .
	manualset3
103623	2	400489	5	NULL	NULL	0	NULL	spins	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In such a system , spins are filtered not only by spin matching-mismatching between both electrodes as in normal spin-valve devices , but also by the orbital symmetry matching-mismatching .
	manualset3
103624	3	400489	5	NULL	NULL	0	NULL	spin matching-mismatching	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In such a system , spins are filtered not only by spin matching-mismatching between both electrodes as in normal spin-valve devices , but also by the orbital symmetry matching-mismatching .
	manualset3
103625	4	400489	5	NULL	NULL	0	NULL	electrodes 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In such a system , spins are filtered not only by spin matching-mismatching between both electrodes as in normal spin-valve devices , but also by the orbital symmetry matching-mismatching .
	manualset3
103626	5	400489	5	NULL	NULL	0	NULL	normal spin-valve devices	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In such a system , spins are filtered not only by spin matching-mismatching between both electrodes as in normal spin-valve devices , but also by the orbital symmetry matching-mismatching .
	manualset3
107682	6	400489	5	NULL	NULL	0	NULL	orbital symmetry matching-mismatching	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In such a system , spins are filtered not only by spin matching-mismatching between both electrodes as in normal spin-valve devices , but also by the orbital symmetry matching-mismatching .
	manualset3
103627	1	400490	5	NULL	NULL	0	NULL	surgical divisions	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In surgical divisions , where you can find the highest percentage of hospital infections , the surgical wounds are definitively the most frequent localization .
	manualset3
103628	2	400490	5	NULL	NULL	0	NULL	highest percentage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In surgical divisions , where you can find the highest percentage of hospital infections , the surgical wounds are definitively the most frequent localization .
	manualset3
103629	3	400490	5	NULL	NULL	0	NULL	hospital infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In surgical divisions , where you can find the highest percentage of hospital infections , the surgical wounds are definitively the most frequent localization .
	manualset3
103630	4	400490	5	NULL	NULL	0	NULL	surgical wounds	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In surgical divisions , where you can find the highest percentage of hospital infections , the surgical wounds are definitively the most frequent localization .
	manualset3
103631	5	400490	5	NULL	NULL	0	NULL	most frequent localization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In surgical divisions , where you can find the highest percentage of hospital infections , the surgical wounds are definitively the most frequent localization .
	manualset3
103632	1	400491	5	NULL	NULL	0	NULL	ten tissue sets	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In ten tissue sets , 2 - to 6-fold higher CYP1B1 expression in peripheral zone as compared to transition zone was observed .
	manualset3
103633	2	400491	5	NULL	NULL	0	NULL	2 - to 6-fold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In ten tissue sets , 2 - to 6-fold higher CYP1B1 expression in peripheral zone as compared to transition zone was observed .
	manualset3
103634	3	400491	5	NULL	NULL	0	NULL	CYP1B1 expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In ten tissue sets , 2 - to 6-fold higher CYP1B1 expression in peripheral zone as compared to transition zone was observed .
	manualset3
103635	4	400491	5	NULL	NULL	0	NULL	peripheral zone	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In ten tissue sets , 2 - to 6-fold higher CYP1B1 expression in peripheral zone as compared to transition zone was observed .
	manualset3
103636	5	400491	5	NULL	NULL	0	NULL	transition zone 	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In ten tissue sets , 2 - to 6-fold higher CYP1B1 expression in peripheral zone as compared to transition zone was observed .
	manualset3
103704	1	400492	5	NULL	NULL	0	NULL	anginal attacks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In terms of anginal attacks , use of beta-adrenergic blockers and nitrates , and exercise performance the surgical group did significantly better than the medical group throughout the 5 years of follow-up , but the difference between the two treatments tended to decrease .
	manualset3
103705	2	400492	5	NULL	NULL	0	NULL	beta-adrenergic blockers	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In terms of anginal attacks , use of beta-adrenergic blockers and nitrates , and exercise performance the surgical group did significantly better than the medical group throughout the 5 years of follow-up , but the difference between the two treatments tended to decrease .
	manualset3
103706	3	400492	5	NULL	NULL	0	NULL	nitrates	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In terms of anginal attacks , use of beta-adrenergic blockers and nitrates , and exercise performance the surgical group did significantly better than the medical group throughout the 5 years of follow-up , but the difference between the two treatments tended to decrease .
	manualset3
103707	4	400492	5	NULL	NULL	0	NULL	exercise performance	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In terms of anginal attacks , use of beta-adrenergic blockers and nitrates , and exercise performance the surgical group did significantly better than the medical group throughout the 5 years of follow-up , but the difference between the two treatments tended to decrease .
	manualset3
103708	5	400492	5	NULL	NULL	0	NULL	surgical group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In terms of anginal attacks , use of beta-adrenergic blockers and nitrates , and exercise performance the surgical group did significantly better than the medical group throughout the 5 years of follow-up , but the difference between the two treatments tended to decrease .
	manualset3
103709	6	400492	5	NULL	NULL	0	NULL	medical group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In terms of anginal attacks , use of beta-adrenergic blockers and nitrates , and exercise performance the surgical group did significantly better than the medical group throughout the 5 years of follow-up , but the difference between the two treatments tended to decrease .
	manualset3
103710	7	400492	5	NULL	NULL	0	NULL	5 years	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In terms of anginal attacks , use of beta-adrenergic blockers and nitrates , and exercise performance the surgical group did significantly better than the medical group throughout the 5 years of follow-up , but the difference between the two treatments tended to decrease .
	manualset3
103711	8	400492	5	NULL	NULL	0	NULL	follow-up	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In terms of anginal attacks , use of beta-adrenergic blockers and nitrates , and exercise performance the surgical group did significantly better than the medical group throughout the 5 years of follow-up , but the difference between the two treatments tended to decrease .
	manualset3
103712	9	400492	5	NULL	NULL	0	NULL	treatments	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In terms of anginal attacks , use of beta-adrenergic blockers and nitrates , and exercise performance the surgical group did significantly better than the medical group throughout the 5 years of follow-up , but the difference between the two treatments tended to decrease .
	manualset3
103713	1	400493	5	NULL	NULL	0	NULL	prophylactic irradiation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In terms of prophylactic irradiation to pelvic lymph nodes , there has been no definitive evidence that prophylactic irradiation of clinically or pathologically uninvolved pelvic lymph nodes improves the overall survival rate .
	manualset3
103714	2	400493	5	NULL	NULL	0	NULL	pelvic lymph nodes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In terms of prophylactic irradiation to pelvic lymph nodes , there has been no definitive evidence that prophylactic irradiation of clinically or pathologically uninvolved pelvic lymph nodes improves the overall survival rate .
	manualset3
103715	3	400493	5	NULL	NULL	0	NULL	definitive evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In terms of prophylactic irradiation to pelvic lymph nodes , there has been no definitive evidence that prophylactic irradiation of clinically or pathologically uninvolved pelvic lymph nodes improves the overall survival rate .
	manualset3
103716	4	400493	5	NULL	NULL	0	NULL	prophylactic irradiation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In terms of prophylactic irradiation to pelvic lymph nodes , there has been no definitive evidence that prophylactic irradiation of clinically or pathologically uninvolved pelvic lymph nodes improves the overall survival rate .
	manualset3
103717	5	400493	5	NULL	NULL	0	NULL	pelvic lymph nodes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In terms of prophylactic irradiation to pelvic lymph nodes , there has been no definitive evidence that prophylactic irradiation of clinically or pathologically uninvolved pelvic lymph nodes improves the overall survival rate .
	manualset3
103718	6	400493	5	NULL	NULL	0	NULL	overall survival rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In terms of prophylactic irradiation to pelvic lymph nodes , there has been no definitive evidence that prophylactic irradiation of clinically or pathologically uninvolved pelvic lymph nodes improves the overall survival rate .
	manualset3
103719	1	400494	5	NULL	NULL	0	NULL	LPA-mediated functional modulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In terms of the LPA-mediated functional modulation of chondrocytes , LPA stimulated cellular proliferation .
	manualset3
103720	2	400494	5	NULL	NULL	0	NULL	chondrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In terms of the LPA-mediated functional modulation of chondrocytes , LPA stimulated cellular proliferation .
	manualset3
103721	3	400494	5	NULL	NULL	0	NULL	LPA stimulated cellular proliferation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In terms of the LPA-mediated functional modulation of chondrocytes , LPA stimulated cellular proliferation .
	manualset3
103722	1	400495	5	NULL	NULL	0	NULL	PIVH	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In that range of PIVH , the outcome was related to the severity of CPVL and not to PIVH grade .
	manualset3
103723	2	400495	5	NULL	NULL	NULL	NULL	outcome	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In that range of PIVH , the outcome was related to the severity of CPVL and not to PIVH grade .
	manualset3
103724	3	400495	5	NULL	NULL	0	NULL	CPVL	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In that range of PIVH , the outcome was related to the severity of CPVL and not to PIVH grade .
	manualset3
103725	4	400495	5	NULL	NULL	0	NULL	PIVH grade	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In that range of PIVH , the outcome was related to the severity of CPVL and not to PIVH grade .
	manualset3
103726	1	400496	5	NULL	NULL	0	NULL	17th century	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 17th century , John Bulwer and George Sibscota , both interested in the deaf and their education , applied the bone conduction phenomenon as an aid to defective hearing .
	manualset3
103727	2	400496	5	NULL	NULL	0	NULL	John Bulwer	person												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 17th century , John Bulwer and George Sibscota , both interested in the deaf and their education , applied the bone conduction phenomenon as an aid to defective hearing .
	manualset3
103728	3	400496	5	NULL	NULL	0	NULL	George Sibscota	person												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 17th century , John Bulwer and George Sibscota , both interested in the deaf and their education , applied the bone conduction phenomenon as an aid to defective hearing .
	manualset3
103729	4	400496	5	NULL	NULL	0	NULL	deaf	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 17th century , John Bulwer and George Sibscota , both interested in the deaf and their education , applied the bone conduction phenomenon as an aid to defective hearing .
	manualset3
103730	5	400496	5	NULL	NULL	0	NULL	education	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 17th century , John Bulwer and George Sibscota , both interested in the deaf and their education , applied the bone conduction phenomenon as an aid to defective hearing .
	manualset3
103731	6	400496	5	NULL	NULL	0	NULL	bone conduction phenomenon	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 17th century , John Bulwer and George Sibscota , both interested in the deaf and their education , applied the bone conduction phenomenon as an aid to defective hearing .
	manualset3
103732	7	400496	5	NULL	NULL	0	NULL	aid	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 17th century , John Bulwer and George Sibscota , both interested in the deaf and their education , applied the bone conduction phenomenon as an aid to defective hearing .
	manualset3
103733	8	400496	5	NULL	NULL	0	NULL	defective hearing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 17th century , John Bulwer and George Sibscota , both interested in the deaf and their education , applied the bone conduction phenomenon as an aid to defective hearing .
	manualset3
103734	1	400497	5	NULL	NULL	0	NULL	1990s	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 1990s regulatory bodies in New Zealand worked to develop guide-lines to clean up the contamination of land caused by the use of pentachlorophenol in the treatment of timber .
	manualset3
103735	2	400497	5	NULL	NULL	0	NULL	regulatory bodies	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 1990s regulatory bodies in New Zealand worked to develop guide-lines to clean up the contamination of land caused by the use of pentachlorophenol in the treatment of timber .
	manualset3
103736	3	400497	5	NULL	NULL	0	NULL	New Zealand 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 1990s regulatory bodies in New Zealand worked to develop guide-lines to clean up the contamination of land caused by the use of pentachlorophenol in the treatment of timber .
	manualset3
103737	4	400497	5	NULL	NULL	0	NULL	guide-lines	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 1990s regulatory bodies in New Zealand worked to develop guide-lines to clean up the contamination of land caused by the use of pentachlorophenol in the treatment of timber .
	manualset3
103738	5	400497	5	NULL	NULL	0	NULL	contamination	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 1990s regulatory bodies in New Zealand worked to develop guide-lines to clean up the contamination of land caused by the use of pentachlorophenol in the treatment of timber .
	manualset3
103739	6	400497	5	NULL	NULL	0	NULL	land	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 1990s regulatory bodies in New Zealand worked to develop guide-lines to clean up the contamination of land caused by the use of pentachlorophenol in the treatment of timber .
	manualset3
103740	7	400497	5	NULL	NULL	0	NULL	pentachlorophenol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 1990s regulatory bodies in New Zealand worked to develop guide-lines to clean up the contamination of land caused by the use of pentachlorophenol in the treatment of timber .
	manualset3
103741	8	400497	5	NULL	NULL	0	NULL	treatment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 1990s regulatory bodies in New Zealand worked to develop guide-lines to clean up the contamination of land caused by the use of pentachlorophenol in the treatment of timber .
	manualset3
103742	9	400497	5	NULL	NULL	0	NULL	timber	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 1990s regulatory bodies in New Zealand worked to develop guide-lines to clean up the contamination of land caused by the use of pentachlorophenol in the treatment of timber .
	manualset3
103743	1	400498	5	NULL	NULL	0	NULL	1st year	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 1st year of operation , new LTCHs relative to existing facilities had fewer occupied beds , shorter length of stay , and lower financial performance .
	manualset3
103744	2	400498	5	NULL	NULL	0	NULL	operation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 1st year of operation , new LTCHs relative to existing facilities had fewer occupied beds , shorter length of stay , and lower financial performance .
	manualset3
103745	3	400498	5	NULL	NULL	0	NULL	new LTCHs	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 1st year of operation , new LTCHs relative to existing facilities had fewer occupied beds , shorter length of stay , and lower financial performance .
	manualset3
103746	4	400498	5	NULL	NULL	0	NULL	existing facilities	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 1st year of operation , new LTCHs relative to existing facilities had fewer occupied beds , shorter length of stay , and lower financial performance .
	manualset3
103747	5	400498	5	NULL	NULL	0	NULL	fewer occupied beds	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 1st year of operation , new LTCHs relative to existing facilities had fewer occupied beds , shorter length of stay , and lower financial performance .
	manualset3
103748	6	400498	5	NULL	NULL	0	NULL	length	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 1st year of operation , new LTCHs relative to existing facilities had fewer occupied beds , shorter length of stay , and lower financial performance .
	manualset3
103749	1	400499	5	NULL	NULL	0	NULL	214 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 214 cases of benign and 103 of malignant ovarian tumors a correct diagnosis was provided by ultrasound in 88 % and 74 % respectively .
	manualset3
103750	2	400499	5	NULL	NULL	0	NULL	benign tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 214 cases of benign and 103 of malignant ovarian tumors a correct diagnosis was provided by ultrasound in 88 % and 74 % respectively .
	manualset3
103751	3	400499	5	NULL	NULL	0	NULL	103	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 214 cases of benign and 103 of malignant ovarian tumors a correct diagnosis was provided by ultrasound in 88 % and 74 % respectively .
	manualset3
103752	4	400499	5	NULL	NULL	0	NULL	malignant ovarian tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 214 cases of benign and 103 of malignant ovarian tumors a correct diagnosis was provided by ultrasound in 88 % and 74 % respectively .
	manualset3
103753	5	400499	5	NULL	NULL	0	NULL	correct diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 214 cases of benign and 103 of malignant ovarian tumors a correct diagnosis was provided by ultrasound in 88 % and 74 % respectively .
	manualset3
103754	6	400499	5	NULL	NULL	0	NULL	ultrasound	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 214 cases of benign and 103 of malignant ovarian tumors a correct diagnosis was provided by ultrasound in 88 % and 74 % respectively .
	manualset3
103755	7	400499	5	NULL	NULL	0	NULL	88 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 214 cases of benign and 103 of malignant ovarian tumors a correct diagnosis was provided by ultrasound in 88 % and 74 % respectively .
	manualset3
103756	8	400499	5	NULL	NULL	0	NULL	74 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 214 cases of benign and 103 of malignant ovarian tumors a correct diagnosis was provided by ultrasound in 88 % and 74 % respectively .
	manualset3
103757	1	400500	5	NULL	NULL	0	NULL	3 year	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 3 year study we observed in the alfacalcidol group as compared with the plain vitamin D group , respectively : a 3 year median percentage increase of BMD at the lumbar spine of 2.4 % versus -0.8 % ( p & lt ; 0.0001 ) ; a median increase at the femoral neck of 1.2 % versus 0.8 % ( p & lt ; 0.006 ) .
	manualset3
103758	2	400500	5	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 3 year study we observed in the alfacalcidol group as compared with the plain vitamin D group , respectively : a 3 year median percentage increase of BMD at the lumbar spine of 2.4 % versus -0.8 % ( p & lt ; 0.0001 ) ; a median increase at the femoral neck of 1.2 % versus 0.8 % ( p & lt ; 0.006 ) .
	manualset3
103759	3	400500	5	NULL	NULL	0	NULL	alfacalcidol group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 3 year study we observed in the alfacalcidol group as compared with the plain vitamin D group , respectively : a 3 year median percentage increase of BMD at the lumbar spine of 2.4 % versus -0.8 % ( p & lt ; 0.0001 ) ; a median increase at the femoral neck of 1.2 % versus 0.8 % ( p & lt ; 0.006 ) .
	manualset3
103760	4	400500	5	NULL	NULL	0	NULL	plain vitamin D group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 3 year study we observed in the alfacalcidol group as compared with the plain vitamin D group , respectively : a 3 year median percentage increase of BMD at the lumbar spine of 2.4 % versus -0.8 % ( p & lt ; 0.0001 ) ; a median increase at the femoral neck of 1.2 % versus 0.8 % ( p & lt ; 0.006 ) .
	manualset3
103761	5	400500	5	NULL	NULL	0	NULL	3 year	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 3 year study we observed in the alfacalcidol group as compared with the plain vitamin D group , respectively : a 3 year median percentage increase of BMD at the lumbar spine of 2.4 % versus -0.8 % ( p & lt ; 0.0001 ) ; a median increase at the femoral neck of 1.2 % versus 0.8 % ( p & lt ; 0.006 ) .
	manualset3
103762	6	400500	5	NULL	NULL	0	NULL	median percentage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 3 year study we observed in the alfacalcidol group as compared with the plain vitamin D group , respectively : a 3 year median percentage increase of BMD at the lumbar spine of 2.4 % versus -0.8 % ( p & lt ; 0.0001 ) ; a median increase at the femoral neck of 1.2 % versus 0.8 % ( p & lt ; 0.006 ) .
	manualset3
103763	7	400500	5	NULL	NULL	0	NULL	BMD	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 3 year study we observed in the alfacalcidol group as compared with the plain vitamin D group , respectively : a 3 year median percentage increase of BMD at the lumbar spine of 2.4 % versus -0.8 % ( p & lt ; 0.0001 ) ; a median increase at the femoral neck of 1.2 % versus 0.8 % ( p & lt ; 0.006 ) .
	manualset3
103764	8	400500	5	NULL	NULL	0	NULL	lumbar spine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 3 year study we observed in the alfacalcidol group as compared with the plain vitamin D group , respectively : a 3 year median percentage increase of BMD at the lumbar spine of 2.4 % versus -0.8 % ( p & lt ; 0.0001 ) ; a median increase at the femoral neck of 1.2 % versus 0.8 % ( p & lt ; 0.006 ) .
	manualset3
103765	9	400500	5	NULL	NULL	0	NULL	2.4 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 3 year study we observed in the alfacalcidol group as compared with the plain vitamin D group , respectively : a 3 year median percentage increase of BMD at the lumbar spine of 2.4 % versus -0.8 % ( p & lt ; 0.0001 ) ; a median increase at the femoral neck of 1.2 % versus 0.8 % ( p & lt ; 0.006 ) .
	manualset3
103766	10	400500	5	NULL	NULL	0	NULL	-0.8 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 3 year study we observed in the alfacalcidol group as compared with the plain vitamin D group , respectively : a 3 year median percentage increase of BMD at the lumbar spine of 2.4 % versus -0.8 % ( p & lt ; 0.0001 ) ; a median increase at the femoral neck of 1.2 % versus 0.8 % ( p & lt ; 0.006 ) .
	manualset3
103767	11	400500	5	NULL	NULL	0	NULL	p & lt ; 0.0001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 3 year study we observed in the alfacalcidol group as compared with the plain vitamin D group , respectively : a 3 year median percentage increase of BMD at the lumbar spine of 2.4 % versus -0.8 % ( p & lt ; 0.0001 ) ; a median increase at the femoral neck of 1.2 % versus 0.8 % ( p & lt ; 0.006 ) .
	manualset3
103768	12	400500	5	NULL	NULL	0	NULL	femoral neck	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 3 year study we observed in the alfacalcidol group as compared with the plain vitamin D group , respectively : a 3 year median percentage increase of BMD at the lumbar spine of 2.4 % versus -0.8 % ( p & lt ; 0.0001 ) ; a median increase at the femoral neck of 1.2 % versus 0.8 % ( p & lt ; 0.006 ) .
	manualset3
103769	13	400500	5	NULL	NULL	0	NULL	1.2 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 3 year study we observed in the alfacalcidol group as compared with the plain vitamin D group , respectively : a 3 year median percentage increase of BMD at the lumbar spine of 2.4 % versus -0.8 % ( p & lt ; 0.0001 ) ; a median increase at the femoral neck of 1.2 % versus 0.8 % ( p & lt ; 0.006 ) .
	manualset3
103770	14	400500	5	NULL	NULL	0	NULL	0.8 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 3 year study we observed in the alfacalcidol group as compared with the plain vitamin D group , respectively : a 3 year median percentage increase of BMD at the lumbar spine of 2.4 % versus -0.8 % ( p & lt ; 0.0001 ) ; a median increase at the femoral neck of 1.2 % versus 0.8 % ( p & lt ; 0.006 ) .
	manualset3
103771	15	400500	5	NULL	NULL	0	NULL	p & lt ; 0.006	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 3 year study we observed in the alfacalcidol group as compared with the plain vitamin D group , respectively : a 3 year median percentage increase of BMD at the lumbar spine of 2.4 % versus -0.8 % ( p & lt ; 0.0001 ) ; a median increase at the femoral neck of 1.2 % versus 0.8 % ( p & lt ; 0.006 ) .
	manualset3
103772	1	400501	5	NULL	NULL	0	NULL	ADX/PNX group	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the ADX/PNX group , MLV was 35 % below that predicted for lung mass. .
	manualset3
103773	2	400501	5	NULL	NULL	0	NULL	MLV	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the ADX/PNX group , MLV was 35 % below that predicted for lung mass. .
	manualset3
103774	3	400501	5	NULL	NULL	0	NULL	35 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the ADX/PNX group , MLV was 35 % below that predicted for lung mass. .
	manualset3
103775	4	400501	5	NULL	NULL	0	NULL	lung mass	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the ADX/PNX group , MLV was 35 % below that predicted for lung mass. .
	manualset3
103776	1	400502	5	NULL	NULL	0	NULL	1 , 5-bis ( dicarboxymethylaminomethyl ) -2 , 6 - dihydroxynaphthalene	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	1 , 5-bis ( dicarboxymethylaminomethyl ) -2 , 6 - dihydroxynaphthalene as a selective spectrofluorimetric reagent for calcium .
	manualset3
103777	2	400502	5	NULL	NULL	0	NULL	spectrofluorimetric reagent	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	1 , 5-bis ( dicarboxymethylaminomethyl ) -2 , 6 - dihydroxynaphthalene as a selective spectrofluorimetric reagent for calcium .
	manualset3
103778	3	400502	5	NULL	NULL	0	NULL	calcium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	1 , 5-bis ( dicarboxymethylaminomethyl ) -2 , 6 - dihydroxynaphthalene as a selective spectrofluorimetric reagent for calcium .
	manualset3
103779	1	400503	5	NULL	NULL	0	NULL	BP fragments	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the BP fragments containing region 43-88 , peptide 1-88 showed the best reactivity , peptide 20-166 showed minimal reactivity , while peptide 1-115 showed none .
	manualset3
103780	2	400503	5	NULL	NULL	0	NULL	region 43-88	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the BP fragments containing region 43-88 , peptide 1-88 showed the best reactivity , peptide 20-166 showed minimal reactivity , while peptide 1-115 showed none .
	manualset3
103781	3	400503	5	NULL	NULL	0	NULL	peptide 1-88	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the BP fragments containing region 43-88 , peptide 1-88 showed the best reactivity , peptide 20-166 showed minimal reactivity , while peptide 1-115 showed none .
	manualset3
103782	4	400503	5	NULL	NULL	0	NULL	peptide 20-166	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the BP fragments containing region 43-88 , peptide 1-88 showed the best reactivity , peptide 20-166 showed minimal reactivity , while peptide 1-115 showed none .
	manualset3
103783	5	400503	5	NULL	NULL	0	NULL	peptide 1-115	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the BP fragments containing region 43-88 , peptide 1-88 showed the best reactivity , peptide 20-166 showed minimal reactivity , while peptide 1-115 showed none .
	manualset3
103784	1	400504	5	NULL	NULL	0	NULL	C ( 4 ) - dominated grasslands	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the C ( 4 ) - dominated grasslands of central North America , a reduction in fire frequency is the most cited cause of this shift in growth forms as fire both enhances grass productivity and constrains the establishment and expansion of native woody vegetation .
	manualset3
103785	2	400504	5	NULL	NULL	0	NULL	central North America	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the C ( 4 ) - dominated grasslands of central North America , a reduction in fire frequency is the most cited cause of this shift in growth forms as fire both enhances grass productivity and constrains the establishment and expansion of native woody vegetation .
	manualset3
103786	3	400504	5	NULL	NULL	0	NULL	fire frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the C ( 4 ) - dominated grasslands of central North America , a reduction in fire frequency is the most cited cause of this shift in growth forms as fire both enhances grass productivity and constrains the establishment and expansion of native woody vegetation .
	manualset3
103787	4	400504	5	NULL	NULL	0	NULL	cause	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the C ( 4 ) - dominated grasslands of central North America , a reduction in fire frequency is the most cited cause of this shift in growth forms as fire both enhances grass productivity and constrains the establishment and expansion of native woody vegetation .
	manualset3
103788	5	400504	5	NULL	NULL	0	NULL	growth forms	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the C ( 4 ) - dominated grasslands of central North America , a reduction in fire frequency is the most cited cause of this shift in growth forms as fire both enhances grass productivity and constrains the establishment and expansion of native woody vegetation .
	manualset3
103789	6	400504	5	NULL	NULL	NULL	NULL	fire	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the C ( 4 ) - dominated grasslands of central North America , a reduction in fire frequency is the most cited cause of this shift in growth forms as fire both enhances grass productivity and constrains the establishment and expansion of native woody vegetation .
	manualset3
103790	7	400504	5	NULL	NULL	NULL	NULL	grass productivity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the C ( 4 ) - dominated grasslands of central North America , a reduction in fire frequency is the most cited cause of this shift in growth forms as fire both enhances grass productivity and constrains the establishment and expansion of native woody vegetation .
	manualset3
103791	8	400504	5	NULL	NULL	NULL	NULL	establishment	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the C ( 4 ) - dominated grasslands of central North America , a reduction in fire frequency is the most cited cause of this shift in growth forms as fire both enhances grass productivity and constrains the establishment and expansion of native woody vegetation .
	manualset3
103792	9	400504	5	NULL	NULL	NULL	NULL	expansion	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the C ( 4 ) - dominated grasslands of central North America , a reduction in fire frequency is the most cited cause of this shift in growth forms as fire both enhances grass productivity and constrains the establishment and expansion of native woody vegetation .
	manualset3
103793	10	400504	5	NULL	NULL	NULL	NULL	native woody vegetation	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the C ( 4 ) - dominated grasslands of central North America , a reduction in fire frequency is the most cited cause of this shift in growth forms as fire both enhances grass productivity and constrains the establishment and expansion of native woody vegetation .
	manualset3
103794	1	400505	5	NULL	NULL	0	NULL	CDL-pancreatitis model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In the CDL-pancreatitis model , after edaravone and vehicle saline were injected intravenously , pancreatitis was induced for 7 h by the CDL technique .
	manualset3
103795	2	400505	5	NULL	NULL	0	NULL	edaravone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the CDL-pancreatitis model , after edaravone and vehicle saline were injected intravenously , pancreatitis was induced for 7 h by the CDL technique .
	manualset3
103796	3	400505	5	NULL	NULL	0	NULL	vehicle saline	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the CDL-pancreatitis model , after edaravone and vehicle saline were injected intravenously , pancreatitis was induced for 7 h by the CDL technique .
	manualset3
103797	4	400505	5	NULL	NULL	0	NULL	pancreatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In the CDL-pancreatitis model , after edaravone and vehicle saline were injected intravenously , pancreatitis was induced for 7 h by the CDL technique .
	manualset3
103798	5	400505	5	NULL	NULL	0	NULL	7 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In the CDL-pancreatitis model , after edaravone and vehicle saline were injected intravenously , pancreatitis was induced for 7 h by the CDL technique .
	manualset3
103799	6	400505	5	NULL	NULL	0	NULL	CDL technique	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the CDL-pancreatitis model , after edaravone and vehicle saline were injected intravenously , pancreatitis was induced for 7 h by the CDL technique .
	manualset3
103800	1	400506	5	NULL	NULL	0	NULL	CLL patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the CLL patients our studies have confirmed the results of the determination of similar parameters by other authors , namely a higher percentage of PAS + lymphocytes than normal together with a variety of humoral and cellular immunity disturbances .
	manualset3
103801	2	400506	5	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the CLL patients our studies have confirmed the results of the determination of similar parameters by other authors , namely a higher percentage of PAS + lymphocytes than normal together with a variety of humoral and cellular immunity disturbances .
	manualset3
103802	3	400506	5	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the CLL patients our studies have confirmed the results of the determination of similar parameters by other authors , namely a higher percentage of PAS + lymphocytes than normal together with a variety of humoral and cellular immunity disturbances .
	manualset3
103803	4	400506	5	NULL	NULL	0	NULL	determination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the CLL patients our studies have confirmed the results of the determination of similar parameters by other authors , namely a higher percentage of PAS + lymphocytes than normal together with a variety of humoral and cellular immunity disturbances .
	manualset3
103804	5	400506	5	NULL	NULL	0	NULL	parameters	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In the CLL patients our studies have confirmed the results of the determination of similar parameters by other authors , namely a higher percentage of PAS + lymphocytes than normal together with a variety of humoral and cellular immunity disturbances .
	manualset3
103805	6	400506	5	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the CLL patients our studies have confirmed the results of the determination of similar parameters by other authors , namely a higher percentage of PAS + lymphocytes than normal together with a variety of humoral and cellular immunity disturbances .
	manualset3
103806	7	400506	5	NULL	NULL	0	NULL	higher percentage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the CLL patients our studies have confirmed the results of the determination of similar parameters by other authors , namely a higher percentage of PAS + lymphocytes than normal together with a variety of humoral and cellular immunity disturbances .
	manualset3
103807	8	400506	5	NULL	NULL	0	NULL	PAS + lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the CLL patients our studies have confirmed the results of the determination of similar parameters by other authors , namely a higher percentage of PAS + lymphocytes than normal together with a variety of humoral and cellular immunity disturbances .
	manualset3
103808	9	400506	5	NULL	NULL	0	NULL	humoral immunity disturbances	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the CLL patients our studies have confirmed the results of the determination of similar parameters by other authors , namely a higher percentage of PAS + lymphocytes than normal together with a variety of humoral and cellular immunity disturbances .
	manualset3
103809	10	400506	5	NULL	NULL	0	NULL	cellular immunity disturbances . 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the CLL patients our studies have confirmed the results of the determination of similar parameters by other authors , namely a higher percentage of PAS + lymphocytes than normal together with a variety of humoral and cellular immunity disturbances .
	manualset3
103810	1	400507	5	NULL	NULL	0	NULL	Coomassie Brilliant Blue G250-assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the Coomassie Brilliant Blue G250-assay 0.10 ml urine are added to 5.0 ml Coomassie Brilliant Blue G250 reagent and the sample is read against the reagent blank .
	manualset3
103811	2	400507	5	NULL	NULL	0	NULL	0.10 ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the Coomassie Brilliant Blue G250-assay 0.10 ml urine are added to 5.0 ml Coomassie Brilliant Blue G250 reagent and the sample is read against the reagent blank .
	manualset3
103812	3	400507	5	NULL	NULL	0	NULL	urine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the Coomassie Brilliant Blue G250-assay 0.10 ml urine are added to 5.0 ml Coomassie Brilliant Blue G250 reagent and the sample is read against the reagent blank .
	manualset3
103813	4	400507	5	NULL	NULL	0	NULL	5.0 ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the Coomassie Brilliant Blue G250-assay 0.10 ml urine are added to 5.0 ml Coomassie Brilliant Blue G250 reagent and the sample is read against the reagent blank .
	manualset3
103814	5	400507	5	NULL	NULL	0	NULL	Coomassie Brilliant Blue G250 reagent	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In the Coomassie Brilliant Blue G250-assay 0.10 ml urine are added to 5.0 ml Coomassie Brilliant Blue G250 reagent and the sample is read against the reagent blank .
	manualset3
103815	6	400507	5	NULL	NULL	0	NULL	sample	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In the Coomassie Brilliant Blue G250-assay 0.10 ml urine are added to 5.0 ml Coomassie Brilliant Blue G250 reagent and the sample is read against the reagent blank .
	manualset3
103816	7	400507	5	NULL	NULL	0	NULL	reagent	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In the Coomassie Brilliant Blue G250-assay 0.10 ml urine are added to 5.0 ml Coomassie Brilliant Blue G250 reagent and the sample is read against the reagent blank .
	manualset3
103817	1	400508	5	NULL	NULL	0	NULL	EI mass spectrum	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the EI mass spectrum , the methyl ester-trimethylsilyl derivative gave characteristic ions at m/z 506 , 462 , 418 , 416 , 328 , 316 , 238 , 228 , 205 , 186 , and 173 .
	manualset3
103818	2	400508	5	NULL	NULL	0	NULL	methyl ester-trimethylsilyl derivative	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the EI mass spectrum , the methyl ester-trimethylsilyl derivative gave characteristic ions at m/z 506 , 462 , 418 , 416 , 328 , 316 , 238 , 228 , 205 , 186 , and 173 .
	manualset3
103819	3	400508	5	NULL	NULL	0	NULL	characteristic ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In the EI mass spectrum , the methyl ester-trimethylsilyl derivative gave characteristic ions at m/z 506 , 462 , 418 , 416 , 328 , 316 , 238 , 228 , 205 , 186 , and 173 .
	manualset3
103820	4	400508	5	NULL	NULL	0	NULL	m/z 506	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the EI mass spectrum , the methyl ester-trimethylsilyl derivative gave characteristic ions at m/z 506 , 462 , 418 , 416 , 328 , 316 , 238 , 228 , 205 , 186 , and 173 .
	manualset3
103821	5	400508	5	NULL	NULL	0	NULL	m/z 462	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the EI mass spectrum , the methyl ester-trimethylsilyl derivative gave characteristic ions at m/z 506 , 462 , 418 , 416 , 328 , 316 , 238 , 228 , 205 , 186 , and 173 .
	manualset3
103822	6	400508	5	NULL	NULL	0	NULL	m/z 418	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the EI mass spectrum , the methyl ester-trimethylsilyl derivative gave characteristic ions at m/z 506 , 462 , 418 , 416 , 328 , 316 , 238 , 228 , 205 , 186 , and 173 .
	manualset3
103823	7	400508	5	NULL	NULL	0	NULL	m/z 416	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the EI mass spectrum , the methyl ester-trimethylsilyl derivative gave characteristic ions at m/z 506 , 462 , 418 , 416 , 328 , 316 , 238 , 228 , 205 , 186 , and 173 .
	manualset3
103824	8	400508	5	NULL	NULL	0	NULL	m/z 328	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the EI mass spectrum , the methyl ester-trimethylsilyl derivative gave characteristic ions at m/z 506 , 462 , 418 , 416 , 328 , 316 , 238 , 228 , 205 , 186 , and 173 .
	manualset3
103825	9	400508	5	NULL	NULL	0	NULL	m/z 316	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the EI mass spectrum , the methyl ester-trimethylsilyl derivative gave characteristic ions at m/z 506 , 462 , 418 , 416 , 328 , 316 , 238 , 228 , 205 , 186 , and 173 .
	manualset3
103826	10	400508	5	NULL	NULL	0	NULL	m/z 238	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the EI mass spectrum , the methyl ester-trimethylsilyl derivative gave characteristic ions at m/z 506 , 462 , 418 , 416 , 328 , 316 , 238 , 228 , 205 , 186 , and 173 .
	manualset3
103827	11	400508	5	NULL	NULL	0	NULL	m/z 228	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the EI mass spectrum , the methyl ester-trimethylsilyl derivative gave characteristic ions at m/z 506 , 462 , 418 , 416 , 328 , 316 , 238 , 228 , 205 , 186 , and 173 .
	manualset3
103828	12	400508	5	NULL	NULL	0	NULL	m/z 205	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the EI mass spectrum , the methyl ester-trimethylsilyl derivative gave characteristic ions at m/z 506 , 462 , 418 , 416 , 328 , 316 , 238 , 228 , 205 , 186 , and 173 .
	manualset3
103829	13	400508	5	NULL	NULL	0	NULL	m/z 186	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the EI mass spectrum , the methyl ester-trimethylsilyl derivative gave characteristic ions at m/z 506 , 462 , 418 , 416 , 328 , 316 , 238 , 228 , 205 , 186 , and 173 .
	manualset3
103830	14	400508	5	NULL	NULL	0	NULL	m/z 173	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the EI mass spectrum , the methyl ester-trimethylsilyl derivative gave characteristic ions at m/z 506 , 462 , 418 , 416 , 328 , 316 , 238 , 228 , 205 , 186 , and 173 .
	manualset3
103831	1	400509	5	NULL	NULL	0	NULL	Eyes category	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In the Eyes category , there were 11 variables describing visual response to stimuli ( e.g. , looking at the observer ) and 10 variables describing appearance of the eyes ( e.g. , glassy , shiny ) .
	manualset3
103832	2	400509	5	NULL	NULL	NULL	NULL	11 variables	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the Eyes category , there were 11 variables describing visual response to stimuli ( e.g. , looking at the observer ) and 10 variables describing appearance of the eyes ( e.g. , glassy , shiny ) .
	manualset3
103833	3	400509	5	NULL	NULL	0	NULL	visual response to stimuli 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the Eyes category , there were 11 variables describing visual response to stimuli ( e.g. , looking at the observer ) and 10 variables describing appearance of the eyes ( e.g. , glassy , shiny ) .
	manualset3
103834	4	400509	5	NULL	NULL	0	NULL	observer	person												NULL		0	NULL	NULL	NULL	NULL	NULL	In the Eyes category , there were 11 variables describing visual response to stimuli ( e.g. , looking at the observer ) and 10 variables describing appearance of the eyes ( e.g. , glassy , shiny ) .
	manualset3
103835	5	400509	5	NULL	NULL	0	NULL	10 variables	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the Eyes category , there were 11 variables describing visual response to stimuli ( e.g. , looking at the observer ) and 10 variables describing appearance of the eyes ( e.g. , glassy , shiny ) .
	manualset3
103836	6	400509	5	NULL	NULL	NULL	NULL	appearance	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the Eyes category , there were 11 variables describing visual response to stimuli ( e.g. , looking at the observer ) and 10 variables describing appearance of the eyes ( e.g. , glassy , shiny ) .
	manualset3
103837	7	400509	5	NULL	NULL	0	NULL	eyes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the Eyes category , there were 11 variables describing visual response to stimuli ( e.g. , looking at the observer ) and 10 variables describing appearance of the eyes ( e.g. , glassy , shiny ) .
	manualset3
103838	1	400510	5	NULL	NULL	0	NULL	GHX group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the GHX group compared with GH rats , media width and CSA were reduced ; in the NX group compared with N rats , media width was increased , lumen decreased and the ratio of media width to lumen diameter increased .
	manualset3
103839	2	400510	5	NULL	NULL	0	NULL	GH rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the GHX group compared with GH rats , media width and CSA were reduced ; in the NX group compared with N rats , media width was increased , lumen decreased and the ratio of media width to lumen diameter increased .
	manualset3
103840	3	400510	5	NULL	NULL	0	NULL	media width	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the GHX group compared with GH rats , media width and CSA were reduced ; in the NX group compared with N rats , media width was increased , lumen decreased and the ratio of media width to lumen diameter increased .
	manualset3
103841	4	400510	5	NULL	NULL	0	NULL	CSA	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the GHX group compared with GH rats , media width and CSA were reduced ; in the NX group compared with N rats , media width was increased , lumen decreased and the ratio of media width to lumen diameter increased .
	manualset3
103842	5	400510	5	NULL	NULL	0	NULL	NX group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the GHX group compared with GH rats , media width and CSA were reduced ; in the NX group compared with N rats , media width was increased , lumen decreased and the ratio of media width to lumen diameter increased .
	manualset3
103843	6	400510	5	NULL	NULL	0	NULL	N rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the GHX group compared with GH rats , media width and CSA were reduced ; in the NX group compared with N rats , media width was increased , lumen decreased and the ratio of media width to lumen diameter increased .
	manualset3
103844	7	400510	5	NULL	NULL	0	NULL	media width	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the GHX group compared with GH rats , media width and CSA were reduced ; in the NX group compared with N rats , media width was increased , lumen decreased and the ratio of media width to lumen diameter increased .
	manualset3
103845	8	400510	5	NULL	NULL	0	NULL	lumen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the GHX group compared with GH rats , media width and CSA were reduced ; in the NX group compared with N rats , media width was increased , lumen decreased and the ratio of media width to lumen diameter increased .
	manualset3
103846	9	400510	5	NULL	NULL	0	NULL	ratio of media width to lumen diameter	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the GHX group compared with GH rats , media width and CSA were reduced ; in the NX group compared with N rats , media width was increased , lumen decreased and the ratio of media width to lumen diameter increased .
	manualset3
103847	1	400511	5	NULL	NULL	0	NULL	H-zone	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the H-zone these changes are consistent with crossbridge changes previously shown by others using freeze-substitution .
	manualset3
103848	2	400511	5	NULL	NULL	0	NULL	changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the H-zone these changes are consistent with crossbridge changes previously shown by others using freeze-substitution .
	manualset3
103849	3	400511	5	NULL	NULL	0	NULL	crossbridge changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the H-zone these changes are consistent with crossbridge changes previously shown by others using freeze-substitution .
	manualset3
103850	4	400511	5	NULL	NULL	0	NULL	freeze-substitution	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the H-zone these changes are consistent with crossbridge changes previously shown by others using freeze-substitution .
	manualset3
103851	1	400512	5	NULL	NULL	NULL	NULL	1 , 5 - and 1 , 7-Azulenequinones	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	1 , 5 - and 1 , 7-Azulenequinones generally showed higher cytotoxicity , as compared with tropolones and azulene derivatives .
	manualset3
103852	2	400512	5	NULL	NULL	0	NULL	cytotoxicity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	1 , 5 - and 1 , 7-Azulenequinones generally showed higher cytotoxicity , as compared with tropolones and azulene derivatives .
	manualset3
103853	3	400512	5	NULL	NULL	0	NULL	tropolones	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	1 , 5 - and 1 , 7-Azulenequinones generally showed higher cytotoxicity , as compared with tropolones and azulene derivatives .
	manualset3
103854	4	400512	5	NULL	NULL	0	NULL	azulene derivatives	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	1 , 5 - and 1 , 7-Azulenequinones generally showed higher cytotoxicity , as compared with tropolones and azulene derivatives .
	manualset3
103855	1	400513	5	NULL	NULL	0	NULL	Japanese series	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the Japanese series conjunctival spheroid degeneration was noticed in 31 % and pinguecula in 60 % , i.e. less frequently than in the sunny Jordan , but more frequently than in Greenland and Denmark .
	manualset3
103856	2	400513	5	NULL	NULL	NULL	NULL	conjunctival spheroid degeneration	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the Japanese series conjunctival spheroid degeneration was noticed in 31 % and pinguecula in 60 % , i.e. less frequently than in the sunny Jordan , but more frequently than in Greenland and Denmark .
	manualset3
103857	3	400513	5	NULL	NULL	0	NULL	31 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the Japanese series conjunctival spheroid degeneration was noticed in 31 % and pinguecula in 60 % , i.e. less frequently than in the sunny Jordan , but more frequently than in Greenland and Denmark .
	manualset3
103858	4	400513	5	NULL	NULL	0	NULL	pinguecula	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In the Japanese series conjunctival spheroid degeneration was noticed in 31 % and pinguecula in 60 % , i.e. less frequently than in the sunny Jordan , but more frequently than in Greenland and Denmark .
	manualset3
103859	5	400513	5	NULL	NULL	0	NULL	60 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the Japanese series conjunctival spheroid degeneration was noticed in 31 % and pinguecula in 60 % , i.e. less frequently than in the sunny Jordan , but more frequently than in Greenland and Denmark .
	manualset3
103860	6	400513	5	NULL	NULL	0	NULL	sunny Jordan	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the Japanese series conjunctival spheroid degeneration was noticed in 31 % and pinguecula in 60 % , i.e. less frequently than in the sunny Jordan , but more frequently than in Greenland and Denmark .
	manualset3
103861	7	400513	5	NULL	NULL	0	NULL	Greenland	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the Japanese series conjunctival spheroid degeneration was noticed in 31 % and pinguecula in 60 % , i.e. less frequently than in the sunny Jordan , but more frequently than in Greenland and Denmark .
	manualset3
103862	8	400513	5	NULL	NULL	0	NULL	Denmark	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the Japanese series conjunctival spheroid degeneration was noticed in 31 % and pinguecula in 60 % , i.e. less frequently than in the sunny Jordan , but more frequently than in Greenland and Denmark .
	manualset3
103863	1	400514	5	NULL	NULL	0	NULL	MS data-dependent workflow	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the MS data-dependent workflow , the goal is to collect as many meaningful spectra as possible by judiciously adjusting the acquisition parameters based on characteristics of the parent masses .
	manualset3
103864	2	400514	5	NULL	NULL	0	NULL	goal	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the MS data-dependent workflow , the goal is to collect as many meaningful spectra as possible by judiciously adjusting the acquisition parameters based on characteristics of the parent masses .
	manualset3
103865	3	400514	5	NULL	NULL	0	NULL	meaningful spectra	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In the MS data-dependent workflow , the goal is to collect as many meaningful spectra as possible by judiciously adjusting the acquisition parameters based on characteristics of the parent masses .
	manualset3
103866	4	400514	5	NULL	NULL	0	NULL	acquisition parameters	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In the MS data-dependent workflow , the goal is to collect as many meaningful spectra as possible by judiciously adjusting the acquisition parameters based on characteristics of the parent masses .
	manualset3
103867	5	400514	5	NULL	NULL	0	NULL	parent masses	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In the MS data-dependent workflow , the goal is to collect as many meaningful spectra as possible by judiciously adjusting the acquisition parameters based on characteristics of the parent masses .
	manualset3
103868	6	400514	5	NULL	NULL	0	NULL	characteristics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the MS data-dependent workflow , the goal is to collect as many meaningful spectra as possible by judiciously adjusting the acquisition parameters based on characteristics of the parent masses .
	manualset3
103869	1	400515	5	NULL	NULL	0	NULL	PACU	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the PACU , coughed secretions are often frankly contaminated with blood , and coughing is unpredictable after airway irritation .
	manualset3
103870	2	400515	5	NULL	NULL	0	NULL	coughed secretions	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the PACU , coughed secretions are often frankly contaminated with blood , and coughing is unpredictable after airway irritation .
	manualset3
103871	3	400515	5	NULL	NULL	0	NULL	blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In the PACU , coughed secretions are often frankly contaminated with blood , and coughing is unpredictable after airway irritation .
	manualset3
103872	4	400515	5	NULL	NULL	0	NULL	coughing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the PACU , coughed secretions are often frankly contaminated with blood , and coughing is unpredictable after airway irritation .
	manualset3
103873	5	400515	5	NULL	NULL	0	NULL	airway irritation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the PACU , coughed secretions are often frankly contaminated with blood , and coughing is unpredictable after airway irritation .
	manualset3
103874	1	400516	5	NULL	NULL	0	NULL	PATH Test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the PATH Test all hypoaesthetic areas could be identified by a reduction of thermal sensitivity .
	manualset3
103875	2	400516	5	NULL	NULL	0	NULL	hypoaesthetic areas	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the PATH Test all hypoaesthetic areas could be identified by a reduction of thermal sensitivity .
	manualset3
103876	3	400516	5	NULL	NULL	0	NULL	thermal sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the PATH Test all hypoaesthetic areas could be identified by a reduction of thermal sensitivity .
	manualset3
103877	1	400517	5	NULL	NULL	0	NULL	PF scenario	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the PF scenario , the resonance state is generally double peaked near the Fermi level , and is abruptly broadened by vortex fluctuations slightly above the transition temperature .
	manualset3
103878	2	400517	5	NULL	NULL	0	NULL	resonance state	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In the PF scenario , the resonance state is generally double peaked near the Fermi level , and is abruptly broadened by vortex fluctuations slightly above the transition temperature .
	manualset3
103879	3	400517	5	NULL	NULL	0	NULL	Fermi level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the PF scenario , the resonance state is generally double peaked near the Fermi level , and is abruptly broadened by vortex fluctuations slightly above the transition temperature .
	manualset3
103880	4	400517	5	NULL	NULL	0	NULL	vortex fluctuations	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In the PF scenario , the resonance state is generally double peaked near the Fermi level , and is abruptly broadened by vortex fluctuations slightly above the transition temperature .
	manualset3
103881	5	400517	5	NULL	NULL	0	NULL	transition temperature	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the PF scenario , the resonance state is generally double peaked near the Fermi level , and is abruptly broadened by vortex fluctuations slightly above the transition temperature .
	manualset3
103882	1	400518	5	NULL	NULL	0	NULL	SD rat liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the SD rat liver , the ductus venosus was therefore established by development of the terminal part of the umbilical vein , which anastomosed directly with the posterior vena cava .
	manualset3
103883	2	400518	5	NULL	NULL	0	NULL	ductus venosus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the SD rat liver , the ductus venosus was therefore established by development of the terminal part of the umbilical vein , which anastomosed directly with the posterior vena cava .
	manualset3
103884	3	400518	5	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the SD rat liver , the ductus venosus was therefore established by development of the terminal part of the umbilical vein , which anastomosed directly with the posterior vena cava .
	manualset3
103885	4	400518	5	NULL	NULL	0	NULL	terminal part of the umbilical vein	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the SD rat liver , the ductus venosus was therefore established by development of the terminal part of the umbilical vein , which anastomosed directly with the posterior vena cava .
	manualset3
103886	5	400518	5	NULL	NULL	0	NULL	posterior vena cava	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the SD rat liver , the ductus venosus was therefore established by development of the terminal part of the umbilical vein , which anastomosed directly with the posterior vena cava .
	manualset3
103887	1	400519	5	NULL	NULL	0	NULL	TNCB-treated sites	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the TNCB-treated sites , marked upregulation of IFN-gamma , IL-1beta , IL-4 , and IL-6 mRNA was observed in addition to B2 receptor mRNA .
	manualset3
103888	2	400519	5	NULL	NULL	0	NULL	upregulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the TNCB-treated sites , marked upregulation of IFN-gamma , IL-1beta , IL-4 , and IL-6 mRNA was observed in addition to B2 receptor mRNA .
	manualset3
103889	3	400519	5	NULL	NULL	0	NULL	IFN-gamma mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the TNCB-treated sites , marked upregulation of IFN-gamma , IL-1beta , IL-4 , and IL-6 mRNA was observed in addition to B2 receptor mRNA .
	manualset3
103890	4	400519	5	NULL	NULL	0	NULL	IL-1beta mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the TNCB-treated sites , marked upregulation of IFN-gamma , IL-1beta , IL-4 , and IL-6 mRNA was observed in addition to B2 receptor mRNA .
	manualset3
103891	5	400519	5	NULL	NULL	0	NULL	IL-4 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the TNCB-treated sites , marked upregulation of IFN-gamma , IL-1beta , IL-4 , and IL-6 mRNA was observed in addition to B2 receptor mRNA .
	manualset3
103892	6	400519	5	NULL	NULL	0	NULL	IL-6 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the TNCB-treated sites , marked upregulation of IFN-gamma , IL-1beta , IL-4 , and IL-6 mRNA was observed in addition to B2 receptor mRNA .
	manualset3
103893	7	400519	5	NULL	NULL	0	NULL	B2 receptor mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the TNCB-treated sites , marked upregulation of IFN-gamma , IL-1beta , IL-4 , and IL-6 mRNA was observed in addition to B2 receptor mRNA .
	manualset3
103894	1	400520	5	NULL	NULL	0	NULL	1 , 990 proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	1 , 990 proteins were predicted to be secreted and to contain signal peptides among 19 , 855 proteins , among which 1 , 936 have SignalPase I signal peptide ( containing 41 with RR-motif signal peptide ) , 53 have SignalPase II signal peptide and one has SignalPase IV signal peptide .
	manualset3
103895	2	400520	5	NULL	NULL	0	NULL	 signal peptides	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	1 , 990 proteins were predicted to be secreted and to contain signal peptides among 19 , 855 proteins , among which 1 , 936 have SignalPase I signal peptide ( containing 41 with RR-motif signal peptide ) , 53 have SignalPase II signal peptide and one has SignalPase IV signal peptide .
	manualset3
103896	3	400520	5	NULL	NULL	0	NULL	19 , 855 proteins	gen												NULL		0	NULL	NULL	NULL	NULL	NULL	1 , 990 proteins were predicted to be secreted and to contain signal peptides among 19 , 855 proteins , among which 1 , 936 have SignalPase I signal peptide ( containing 41 with RR-motif signal peptide ) , 53 have SignalPase II signal peptide and one has SignalPase IV signal peptide .
	manualset3
103897	4	400520	5	NULL	NULL	0	NULL	1 , 936	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	1 , 990 proteins were predicted to be secreted and to contain signal peptides among 19 , 855 proteins , among which 1 , 936 have SignalPase I signal peptide ( containing 41 with RR-motif signal peptide ) , 53 have SignalPase II signal peptide and one has SignalPase IV signal peptide .
	manualset3
103898	5	400520	5	NULL	NULL	0	NULL	SignalPase I signal peptide	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	1 , 990 proteins were predicted to be secreted and to contain signal peptides among 19 , 855 proteins , among which 1 , 936 have SignalPase I signal peptide ( containing 41 with RR-motif signal peptide ) , 53 have SignalPase II signal peptide and one has SignalPase IV signal peptide .
	manualset3
103899	6	400520	5	NULL	NULL	0	NULL	41	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	1 , 990 proteins were predicted to be secreted and to contain signal peptides among 19 , 855 proteins , among which 1 , 936 have SignalPase I signal peptide ( containing 41 with RR-motif signal peptide ) , 53 have SignalPase II signal peptide and one has SignalPase IV signal peptide .
	manualset3
103900	7	400520	5	NULL	NULL	0	NULL	RR-motif signal peptide	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	1 , 990 proteins were predicted to be secreted and to contain signal peptides among 19 , 855 proteins , among which 1 , 936 have SignalPase I signal peptide ( containing 41 with RR-motif signal peptide ) , 53 have SignalPase II signal peptide and one has SignalPase IV signal peptide .
	manualset3
103901	8	400520	5	NULL	NULL	0	NULL	53	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	1 , 990 proteins were predicted to be secreted and to contain signal peptides among 19 , 855 proteins , among which 1 , 936 have SignalPase I signal peptide ( containing 41 with RR-motif signal peptide ) , 53 have SignalPase II signal peptide and one has SignalPase IV signal peptide .
	manualset3
103902	9	400520	5	NULL	NULL	0	NULL	SignalPase II signal peptide	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	1 , 990 proteins were predicted to be secreted and to contain signal peptides among 19 , 855 proteins , among which 1 , 936 have SignalPase I signal peptide ( containing 41 with RR-motif signal peptide ) , 53 have SignalPase II signal peptide and one has SignalPase IV signal peptide .
	manualset3
103903	10	400520	5	NULL	NULL	0	NULL	SignalPase IV signal peptide	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	1 , 990 proteins were predicted to be secreted and to contain signal peptides among 19 , 855 proteins , among which 1 , 936 have SignalPase I signal peptide ( containing 41 with RR-motif signal peptide ) , 53 have SignalPase II signal peptide and one has SignalPase IV signal peptide .
	manualset3
103904	1	400521	5	NULL	NULL	0	NULL	UK	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the UK , where T2 * measurement was first used in the clinical care of patients with thalassemia major , a large and significant fall in mortality has been seen in this patient group .
	manualset3
103905	2	400521	5	NULL	NULL	0	NULL	T2 * measurement	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the UK , where T2 * measurement was first used in the clinical care of patients with thalassemia major , a large and significant fall in mortality has been seen in this patient group .
	manualset3
103906	3	400521	5	NULL	NULL	0	NULL	clinical care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the UK , where T2 * measurement was first used in the clinical care of patients with thalassemia major , a large and significant fall in mortality has been seen in this patient group .
	manualset3
103907	4	400521	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the UK , where T2 * measurement was first used in the clinical care of patients with thalassemia major , a large and significant fall in mortality has been seen in this patient group .
	manualset3
103908	5	400521	5	NULL	NULL	0	NULL	thalassemia major	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In the UK , where T2 * measurement was first used in the clinical care of patients with thalassemia major , a large and significant fall in mortality has been seen in this patient group .
	manualset3
103909	6	400521	5	NULL	NULL	0	NULL	large and significant fall	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the UK , where T2 * measurement was first used in the clinical care of patients with thalassemia major , a large and significant fall in mortality has been seen in this patient group .
	manualset3
103910	7	400521	5	NULL	NULL	0	NULL	mortality	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the UK , where T2 * measurement was first used in the clinical care of patients with thalassemia major , a large and significant fall in mortality has been seen in this patient group .
	manualset3
103911	8	400521	5	NULL	NULL	0	NULL	patient group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the UK , where T2 * measurement was first used in the clinical care of patients with thalassemia major , a large and significant fall in mortality has been seen in this patient group .
	manualset3
103912	1	400522	5	NULL	NULL	0	NULL	USA	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the USA , the National Committee for Clinical Laboratory Standards has studied and published a reference agar dilution method for the susceptibility testing of anaerobic bacteria .
	manualset3
103913	2	400522	5	NULL	NULL	0	NULL	National Committee for Clinical Laboratory Standards	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the USA , the National Committee for Clinical Laboratory Standards has studied and published a reference agar dilution method for the susceptibility testing of anaerobic bacteria .
	manualset3
103914	3	400522	5	NULL	NULL	0	NULL	reference agar dilution method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In the USA , the National Committee for Clinical Laboratory Standards has studied and published a reference agar dilution method for the susceptibility testing of anaerobic bacteria .
	manualset3
103915	4	400522	5	NULL	NULL	0	NULL	susceptibility testing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the USA , the National Committee for Clinical Laboratory Standards has studied and published a reference agar dilution method for the susceptibility testing of anaerobic bacteria .
	manualset3
103916	5	400522	5	NULL	NULL	0	NULL	anaerobic bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the USA , the National Committee for Clinical Laboratory Standards has studied and published a reference agar dilution method for the susceptibility testing of anaerobic bacteria .
	manualset3
103917	1	400523	5	NULL	NULL	0	NULL	United States	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the United States , many tuberculosis patients are treated under government health system with DOT .
	manualset3
103918	2	400523	5	NULL	NULL	0	NULL	tuberculosis patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the United States , many tuberculosis patients are treated under government health system with DOT .
	manualset3
103919	3	400523	5	NULL	NULL	0	NULL	government health system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In the United States , many tuberculosis patients are treated under government health system with DOT .
	manualset3
103920	4	400523	5	NULL	NULL	0	NULL	DOT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the United States , many tuberculosis patients are treated under government health system with DOT .
	manualset3
103921	1	400524	5	NULL	NULL	0	NULL	abdominal cavity	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the abdominal cavity , leukocyte infiltrates were significantly greater in FGN-injected ( 8 h ) and SE/FGN-injected ( 4 and 24 h ) birds than in the SE-injected control birds .
	manualset3
103922	2	400524	5	NULL	NULL	0	NULL	leukocyte infiltrates	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the abdominal cavity , leukocyte infiltrates were significantly greater in FGN-injected ( 8 h ) and SE/FGN-injected ( 4 and 24 h ) birds than in the SE-injected control birds .
	manualset3
103923	3	400524	5	NULL	NULL	0	NULL	FGN-injected birds	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the abdominal cavity , leukocyte infiltrates were significantly greater in FGN-injected ( 8 h ) and SE/FGN-injected ( 4 and 24 h ) birds than in the SE-injected control birds .
	manualset3
103924	4	400524	5	NULL	NULL	0	NULL	8 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In the abdominal cavity , leukocyte infiltrates were significantly greater in FGN-injected ( 8 h ) and SE/FGN-injected ( 4 and 24 h ) birds than in the SE-injected control birds .
	manualset3
103925	5	400524	5	NULL	NULL	0	NULL	SE/FGN-injected birds	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the abdominal cavity , leukocyte infiltrates were significantly greater in FGN-injected ( 8 h ) and SE/FGN-injected ( 4 and 24 h ) birds than in the SE-injected control birds .
	manualset3
103926	6	400524	5	NULL	NULL	0	NULL	4 and 24 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In the abdominal cavity , leukocyte infiltrates were significantly greater in FGN-injected ( 8 h ) and SE/FGN-injected ( 4 and 24 h ) birds than in the SE-injected control birds .
	manualset3
103927	7	400524	5	NULL	NULL	0	NULL	SE-injected control birds	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the abdominal cavity , leukocyte infiltrates were significantly greater in FGN-injected ( 8 h ) and SE/FGN-injected ( 4 and 24 h ) birds than in the SE-injected control birds .
	manualset3
103928	1	400525	5	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of 2a , 1a stabilized RNA2 and induced RNA2 to associate with membrane .
	manualset3
103929	2	400525	5	NULL	NULL	NULL	NULL	2a	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the absence of 2a , 1a stabilized RNA2 and induced RNA2 to associate with membrane .
	manualset3
103930	3	400525	5	NULL	NULL	0	NULL	1a	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of 2a , 1a stabilized RNA2 and induced RNA2 to associate with membrane .
	manualset3
103931	4	400525	5	NULL	NULL	0	NULL	RNA2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of 2a , 1a stabilized RNA2 and induced RNA2 to associate with membrane .
	manualset3
103932	5	400525	5	NULL	NULL	0	NULL	RNA2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of 2a , 1a stabilized RNA2 and induced RNA2 to associate with membrane .
	manualset3
103933	6	400525	5	NULL	NULL	0	NULL	membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of 2a , 1a stabilized RNA2 and induced RNA2 to associate with membrane .
	manualset3
103934	1	400526	5	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of AT ( 2 ) receptor transcription , we found increased AT ( 1 ) receptor binding in brain areas involved in the regulation of the hypothalamic-pituitary-adrenal axis , the hypothalamic paraventricular nucleus and the median eminence , and increased adrenal catecholamine synthesis as shown by higher adrenomedullary tyrosine hydroxylase mRNA and higher adrenal dopamine , norepinephrine and epinephrine levels when compared to wild-type mice .
	manualset3
103935	2	400526	5	NULL	NULL	0	NULL	AT ( 2 ) receptor transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of AT ( 2 ) receptor transcription , we found increased AT ( 1 ) receptor binding in brain areas involved in the regulation of the hypothalamic-pituitary-adrenal axis , the hypothalamic paraventricular nucleus and the median eminence , and increased adrenal catecholamine synthesis as shown by higher adrenomedullary tyrosine hydroxylase mRNA and higher adrenal dopamine , norepinephrine and epinephrine levels when compared to wild-type mice .
	manualset3
103936	3	400526	5	NULL	NULL	0	NULL	AT ( 1 ) receptor binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of AT ( 2 ) receptor transcription , we found increased AT ( 1 ) receptor binding in brain areas involved in the regulation of the hypothalamic-pituitary-adrenal axis , the hypothalamic paraventricular nucleus and the median eminence , and increased adrenal catecholamine synthesis as shown by higher adrenomedullary tyrosine hydroxylase mRNA and higher adrenal dopamine , norepinephrine and epinephrine levels when compared to wild-type mice .
	manualset3
103937	4	400526	5	NULL	NULL	0	NULL	brain areas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of AT ( 2 ) receptor transcription , we found increased AT ( 1 ) receptor binding in brain areas involved in the regulation of the hypothalamic-pituitary-adrenal axis , the hypothalamic paraventricular nucleus and the median eminence , and increased adrenal catecholamine synthesis as shown by higher adrenomedullary tyrosine hydroxylase mRNA and higher adrenal dopamine , norepinephrine and epinephrine levels when compared to wild-type mice .
	manualset3
103938	5	400526	5	NULL	NULL	0	NULL	regulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of AT ( 2 ) receptor transcription , we found increased AT ( 1 ) receptor binding in brain areas involved in the regulation of the hypothalamic-pituitary-adrenal axis , the hypothalamic paraventricular nucleus and the median eminence , and increased adrenal catecholamine synthesis as shown by higher adrenomedullary tyrosine hydroxylase mRNA and higher adrenal dopamine , norepinephrine and epinephrine levels when compared to wild-type mice .
	manualset3
103939	6	400526	5	NULL	NULL	0	NULL	hypothalamic-pituitary-adrenal axis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of AT ( 2 ) receptor transcription , we found increased AT ( 1 ) receptor binding in brain areas involved in the regulation of the hypothalamic-pituitary-adrenal axis , the hypothalamic paraventricular nucleus and the median eminence , and increased adrenal catecholamine synthesis as shown by higher adrenomedullary tyrosine hydroxylase mRNA and higher adrenal dopamine , norepinephrine and epinephrine levels when compared to wild-type mice .
	manualset3
103940	7	400526	5	NULL	NULL	0	NULL	hypothalamic paraventricular nucleus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of AT ( 2 ) receptor transcription , we found increased AT ( 1 ) receptor binding in brain areas involved in the regulation of the hypothalamic-pituitary-adrenal axis , the hypothalamic paraventricular nucleus and the median eminence , and increased adrenal catecholamine synthesis as shown by higher adrenomedullary tyrosine hydroxylase mRNA and higher adrenal dopamine , norepinephrine and epinephrine levels when compared to wild-type mice .
	manualset3
103941	8	400526	5	NULL	NULL	0	NULL	median eminence	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of AT ( 2 ) receptor transcription , we found increased AT ( 1 ) receptor binding in brain areas involved in the regulation of the hypothalamic-pituitary-adrenal axis , the hypothalamic paraventricular nucleus and the median eminence , and increased adrenal catecholamine synthesis as shown by higher adrenomedullary tyrosine hydroxylase mRNA and higher adrenal dopamine , norepinephrine and epinephrine levels when compared to wild-type mice .
	manualset3
103942	9	400526	5	NULL	NULL	0	NULL	increased adrenal catecholamine synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of AT ( 2 ) receptor transcription , we found increased AT ( 1 ) receptor binding in brain areas involved in the regulation of the hypothalamic-pituitary-adrenal axis , the hypothalamic paraventricular nucleus and the median eminence , and increased adrenal catecholamine synthesis as shown by higher adrenomedullary tyrosine hydroxylase mRNA and higher adrenal dopamine , norepinephrine and epinephrine levels when compared to wild-type mice .
	manualset3
103943	10	400526	5	NULL	NULL	0	NULL	adrenomedullary tyrosine hydroxylase mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of AT ( 2 ) receptor transcription , we found increased AT ( 1 ) receptor binding in brain areas involved in the regulation of the hypothalamic-pituitary-adrenal axis , the hypothalamic paraventricular nucleus and the median eminence , and increased adrenal catecholamine synthesis as shown by higher adrenomedullary tyrosine hydroxylase mRNA and higher adrenal dopamine , norepinephrine and epinephrine levels when compared to wild-type mice .
	manualset3
103944	11	400526	5	NULL	NULL	0	NULL	adrenal dopamine level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of AT ( 2 ) receptor transcription , we found increased AT ( 1 ) receptor binding in brain areas involved in the regulation of the hypothalamic-pituitary-adrenal axis , the hypothalamic paraventricular nucleus and the median eminence , and increased adrenal catecholamine synthesis as shown by higher adrenomedullary tyrosine hydroxylase mRNA and higher adrenal dopamine , norepinephrine and epinephrine levels when compared to wild-type mice .
	manualset3
103945	12	400526	5	NULL	NULL	0	NULL	norepinephrine level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of AT ( 2 ) receptor transcription , we found increased AT ( 1 ) receptor binding in brain areas involved in the regulation of the hypothalamic-pituitary-adrenal axis , the hypothalamic paraventricular nucleus and the median eminence , and increased adrenal catecholamine synthesis as shown by higher adrenomedullary tyrosine hydroxylase mRNA and higher adrenal dopamine , norepinephrine and epinephrine levels when compared to wild-type mice .
	manualset3
103946	13	400526	5	NULL	NULL	0	NULL	epinephrine levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of AT ( 2 ) receptor transcription , we found increased AT ( 1 ) receptor binding in brain areas involved in the regulation of the hypothalamic-pituitary-adrenal axis , the hypothalamic paraventricular nucleus and the median eminence , and increased adrenal catecholamine synthesis as shown by higher adrenomedullary tyrosine hydroxylase mRNA and higher adrenal dopamine , norepinephrine and epinephrine levels when compared to wild-type mice .
	manualset3
103947	14	400526	5	NULL	NULL	0	NULL	wild-type mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of AT ( 2 ) receptor transcription , we found increased AT ( 1 ) receptor binding in brain areas involved in the regulation of the hypothalamic-pituitary-adrenal axis , the hypothalamic paraventricular nucleus and the median eminence , and increased adrenal catecholamine synthesis as shown by higher adrenomedullary tyrosine hydroxylase mRNA and higher adrenal dopamine , norepinephrine and epinephrine levels when compared to wild-type mice .
	manualset3
103948	1	400527	5	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of IL-3 , cells still complete the repair of DNA breaks within 15 min , and continue to cycle for 5 h. At this time , IL-3 is necessary to prevent the accelerated onset of DNA cleavage from a G2 arrest point .
	manualset3
103949	2	400527	5	NULL	NULL	0	NULL	IL-3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of IL-3 , cells still complete the repair of DNA breaks within 15 min , and continue to cycle for 5 h. At this time , IL-3 is necessary to prevent the accelerated onset of DNA cleavage from a G2 arrest point .
	manualset3
103950	3	400527	5	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of IL-3 , cells still complete the repair of DNA breaks within 15 min , and continue to cycle for 5 h. At this time , IL-3 is necessary to prevent the accelerated onset of DNA cleavage from a G2 arrest point .
	manualset3
103951	4	400527	5	NULL	NULL	NULL	NULL	repair of DNA breaks	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the absence of IL-3 , cells still complete the repair of DNA breaks within 15 min , and continue to cycle for 5 h. At this time , IL-3 is necessary to prevent the accelerated onset of DNA cleavage from a G2 arrest point .
	manualset3
103952	5	400527	5	NULL	NULL	0	NULL	15 min	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of IL-3 , cells still complete the repair of DNA breaks within 15 min , and continue to cycle for 5 h. At this time , IL-3 is necessary to prevent the accelerated onset of DNA cleavage from a G2 arrest point .
	manualset3
103953	6	400527	5	NULL	NULL	0	NULL	cycle	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of IL-3 , cells still complete the repair of DNA breaks within 15 min , and continue to cycle for 5 h. At this time , IL-3 is necessary to prevent the accelerated onset of DNA cleavage from a G2 arrest point .
	manualset3
103954	7	400527	5	NULL	NULL	0	NULL	5 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of IL-3 , cells still complete the repair of DNA breaks within 15 min , and continue to cycle for 5 h. At this time , IL-3 is necessary to prevent the accelerated onset of DNA cleavage from a G2 arrest point .
	manualset3
103955	8	400527	5	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of IL-3 , cells still complete the repair of DNA breaks within 15 min , and continue to cycle for 5 h. At this time , IL-3 is necessary to prevent the accelerated onset of DNA cleavage from a G2 arrest point .
	manualset3
103956	9	400527	5	NULL	NULL	0	NULL	IL-3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of IL-3 , cells still complete the repair of DNA breaks within 15 min , and continue to cycle for 5 h. At this time , IL-3 is necessary to prevent the accelerated onset of DNA cleavage from a G2 arrest point .
	manualset3
103957	10	400527	5	NULL	NULL	0	NULL	DNA cleavage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of IL-3 , cells still complete the repair of DNA breaks within 15 min , and continue to cycle for 5 h. At this time , IL-3 is necessary to prevent the accelerated onset of DNA cleavage from a G2 arrest point .
	manualset3
103958	11	400527	5	NULL	NULL	0	NULL	G2 arrest point	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of IL-3 , cells still complete the repair of DNA breaks within 15 min , and continue to cycle for 5 h. At this time , IL-3 is necessary to prevent the accelerated onset of DNA cleavage from a G2 arrest point .
	manualset3
103959	1	400528	5	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of PTH , HC diminished the TmPi from 8.36 to 6.58 mumol/min ( P less than 0.005 ) and the TmPi/GFR from 3.36 to 2.51 mumol/ml ( P less than 0.001 ) .
	manualset3
103960	2	400528	5	NULL	NULL	0	NULL	PTH 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of PTH , HC diminished the TmPi from 8.36 to 6.58 mumol/min ( P less than 0.005 ) and the TmPi/GFR from 3.36 to 2.51 mumol/ml ( P less than 0.001 ) .
	manualset3
103961	3	400528	5	NULL	NULL	0	NULL	HC	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of PTH , HC diminished the TmPi from 8.36 to 6.58 mumol/min ( P less than 0.005 ) and the TmPi/GFR from 3.36 to 2.51 mumol/ml ( P less than 0.001 ) .
	manualset3
103962	4	400528	5	NULL	NULL	0	NULL	TmPi	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of PTH , HC diminished the TmPi from 8.36 to 6.58 mumol/min ( P less than 0.005 ) and the TmPi/GFR from 3.36 to 2.51 mumol/ml ( P less than 0.001 ) .
	manualset3
103963	5	400528	5	NULL	NULL	0	NULL	8.36 mumol/min	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of PTH , HC diminished the TmPi from 8.36 to 6.58 mumol/min ( P less than 0.005 ) and the TmPi/GFR from 3.36 to 2.51 mumol/ml ( P less than 0.001 ) .
	manualset3
103964	6	400528	5	NULL	NULL	0	NULL	6.58 mumol/min	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of PTH , HC diminished the TmPi from 8.36 to 6.58 mumol/min ( P less than 0.005 ) and the TmPi/GFR from 3.36 to 2.51 mumol/ml ( P less than 0.001 ) .
	manualset3
103965	7	400528	5	NULL	NULL	0	NULL	P less than 0.005	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of PTH , HC diminished the TmPi from 8.36 to 6.58 mumol/min ( P less than 0.005 ) and the TmPi/GFR from 3.36 to 2.51 mumol/ml ( P less than 0.001 ) .
	manualset3
103966	8	400528	5	NULL	NULL	0	NULL	TmPi/GFR 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of PTH , HC diminished the TmPi from 8.36 to 6.58 mumol/min ( P less than 0.005 ) and the TmPi/GFR from 3.36 to 2.51 mumol/ml ( P less than 0.001 ) .
	manualset3
103967	9	400528	5	NULL	NULL	0	NULL	3.36 mumol/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of PTH , HC diminished the TmPi from 8.36 to 6.58 mumol/min ( P less than 0.005 ) and the TmPi/GFR from 3.36 to 2.51 mumol/ml ( P less than 0.001 ) .
	manualset3
103968	10	400528	5	NULL	NULL	0	NULL	2.51 mumol/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of PTH , HC diminished the TmPi from 8.36 to 6.58 mumol/min ( P less than 0.005 ) and the TmPi/GFR from 3.36 to 2.51 mumol/ml ( P less than 0.001 ) .
	manualset3
103969	11	400528	5	NULL	NULL	0	NULL	P less than 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of PTH , HC diminished the TmPi from 8.36 to 6.58 mumol/min ( P less than 0.005 ) and the TmPi/GFR from 3.36 to 2.51 mumol/ml ( P less than 0.001 ) .
	manualset3
103970	1	400529	5	NULL	NULL	0	NULL	absence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of fever , PGE2 was usually below the threshold of the assay ( 0.05-0 .37 ng/ml ) , while TXB2 was measurable in the majority of cases and its concentration was greater in the third ventricle ( about 0.7 ng/ml ) than in the cisterna magna ( about 0.2 ng/ml ) .
	manualset3
103971	2	400529	5	NULL	NULL	0	NULL	fever 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of fever , PGE2 was usually below the threshold of the assay ( 0.05-0 .37 ng/ml ) , while TXB2 was measurable in the majority of cases and its concentration was greater in the third ventricle ( about 0.7 ng/ml ) than in the cisterna magna ( about 0.2 ng/ml ) .
	manualset3
103972	3	400529	5	NULL	NULL	NULL	NULL	PGE2	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the absence of fever , PGE2 was usually below the threshold of the assay ( 0.05-0 .37 ng/ml ) , while TXB2 was measurable in the majority of cases and its concentration was greater in the third ventricle ( about 0.7 ng/ml ) than in the cisterna magna ( about 0.2 ng/ml ) .
	manualset3
103973	4	400529	5	NULL	NULL	0	NULL	threshold 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of fever , PGE2 was usually below the threshold of the assay ( 0.05-0 .37 ng/ml ) , while TXB2 was measurable in the majority of cases and its concentration was greater in the third ventricle ( about 0.7 ng/ml ) than in the cisterna magna ( about 0.2 ng/ml ) .
	manualset3
103974	5	400529	5	NULL	NULL	0	NULL	assay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of fever , PGE2 was usually below the threshold of the assay ( 0.05-0 .37 ng/ml ) , while TXB2 was measurable in the majority of cases and its concentration was greater in the third ventricle ( about 0.7 ng/ml ) than in the cisterna magna ( about 0.2 ng/ml ) .
	manualset3
103975	6	400529	5	NULL	NULL	0	NULL	0.05-0 .37 ng/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of fever , PGE2 was usually below the threshold of the assay ( 0.05-0 .37 ng/ml ) , while TXB2 was measurable in the majority of cases and its concentration was greater in the third ventricle ( about 0.7 ng/ml ) than in the cisterna magna ( about 0.2 ng/ml ) .
	manualset3
103976	7	400529	5	NULL	NULL	0	NULL	TXB2	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of fever , PGE2 was usually below the threshold of the assay ( 0.05-0 .37 ng/ml ) , while TXB2 was measurable in the majority of cases and its concentration was greater in the third ventricle ( about 0.7 ng/ml ) than in the cisterna magna ( about 0.2 ng/ml ) .
	manualset3
103977	8	400529	5	NULL	NULL	0	NULL	cases 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of fever , PGE2 was usually below the threshold of the assay ( 0.05-0 .37 ng/ml ) , while TXB2 was measurable in the majority of cases and its concentration was greater in the third ventricle ( about 0.7 ng/ml ) than in the cisterna magna ( about 0.2 ng/ml ) .
	manualset3
103978	9	400529	5	NULL	NULL	0	NULL	concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of fever , PGE2 was usually below the threshold of the assay ( 0.05-0 .37 ng/ml ) , while TXB2 was measurable in the majority of cases and its concentration was greater in the third ventricle ( about 0.7 ng/ml ) than in the cisterna magna ( about 0.2 ng/ml ) .
	manualset3
103979	10	400529	5	NULL	NULL	0	NULL	third ventricle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of fever , PGE2 was usually below the threshold of the assay ( 0.05-0 .37 ng/ml ) , while TXB2 was measurable in the majority of cases and its concentration was greater in the third ventricle ( about 0.7 ng/ml ) than in the cisterna magna ( about 0.2 ng/ml ) .
	manualset3
103980	11	400529	5	NULL	NULL	0	NULL	0.7 ng/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of fever , PGE2 was usually below the threshold of the assay ( 0.05-0 .37 ng/ml ) , while TXB2 was measurable in the majority of cases and its concentration was greater in the third ventricle ( about 0.7 ng/ml ) than in the cisterna magna ( about 0.2 ng/ml ) .
	manualset3
103981	12	400529	5	NULL	NULL	0	NULL	cisterna magna	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of fever , PGE2 was usually below the threshold of the assay ( 0.05-0 .37 ng/ml ) , while TXB2 was measurable in the majority of cases and its concentration was greater in the third ventricle ( about 0.7 ng/ml ) than in the cisterna magna ( about 0.2 ng/ml ) .
	manualset3
103982	13	400529	5	NULL	NULL	0	NULL	0.2 ng/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of fever , PGE2 was usually below the threshold of the assay ( 0.05-0 .37 ng/ml ) , while TXB2 was measurable in the majority of cases and its concentration was greater in the third ventricle ( about 0.7 ng/ml ) than in the cisterna magna ( about 0.2 ng/ml ) .
	manualset3
103983	1	400530	5	NULL	NULL	NULL	NULL	1-Carboxymethyl-3-hydroxy-2-methyl-4-pyridone	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	1-Carboxymethyl-3-hydroxy-2-methyl-4-pyridone is obtained from isomaltol and glycine .
	manualset3
103984	2	400530	5	NULL	NULL	0	NULL	isomaltol 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	1-Carboxymethyl-3-hydroxy-2-methyl-4-pyridone is obtained from isomaltol and glycine .
	manualset3
103985	3	400530	5	NULL	NULL	0	NULL	glycine 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	1-Carboxymethyl-3-hydroxy-2-methyl-4-pyridone is obtained from isomaltol and glycine .
	manualset3
94188	1	400531	13	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of mitogens , dietary ascorbyl-2-phosphate increased basal 3H-methyl thymidine incorporation by cultured lymphocytes .
	manualset3
94189	2	400531	13	NULL	NULL	0	NULL	mitogens	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of mitogens , dietary ascorbyl-2-phosphate increased basal 3H-methyl thymidine incorporation by cultured lymphocytes .
	manualset3
94190	3	400531	13	NULL	NULL	0	NULL	dietary ascorbyl-2-phosphate	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of mitogens , dietary ascorbyl-2-phosphate increased basal 3H-methyl thymidine incorporation by cultured lymphocytes .
	manualset3
94191	4	400531	13	NULL	NULL	0	NULL	basal 3H-methyl thymidine incorporation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of mitogens , dietary ascorbyl-2-phosphate increased basal 3H-methyl thymidine incorporation by cultured lymphocytes .
	manualset3
94192	5	400531	13	NULL	NULL	0	NULL	cultured lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of mitogens , dietary ascorbyl-2-phosphate increased basal 3H-methyl thymidine incorporation by cultured lymphocytes .
	manualset3
94193	1	400532	13	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of oestradiol , 4OHT but not ICI 182780 caused significant stimulation of colony formation at low ( 0.01-1 .00 nM ) concentrations .
	manualset3
94194	2	400532	13	NULL	NULL	0	NULL	oestradiol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of oestradiol , 4OHT but not ICI 182780 caused significant stimulation of colony formation at low ( 0.01-1 .00 nM ) concentrations .
	manualset3
94195	3	400532	13	NULL	NULL	0	NULL	 4OHT	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of oestradiol , 4OHT but not ICI 182780 caused significant stimulation of colony formation at low ( 0.01-1 .00 nM ) concentrations .
	manualset3
94196	4	400532	13	NULL	NULL	0	NULL	ICI 182780	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of oestradiol , 4OHT but not ICI 182780 caused significant stimulation of colony formation at low ( 0.01-1 .00 nM ) concentrations .
	manualset3
94197	5	400532	13	NULL	NULL	NULL	NULL	stimulation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the absence of oestradiol , 4OHT but not ICI 182780 caused significant stimulation of colony formation at low ( 0.01-1 .00 nM ) concentrations .
	manualset3
94198	6	400532	13	NULL	NULL	0	NULL	colony formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of oestradiol , 4OHT but not ICI 182780 caused significant stimulation of colony formation at low ( 0.01-1 .00 nM ) concentrations .
	manualset3
94199	7	400532	13	NULL	NULL	0	NULL	low ( 0.01-1 .00 nM ) concentrations	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of oestradiol , 4OHT but not ICI 182780 caused significant stimulation of colony formation at low ( 0.01-1 .00 nM ) concentrations .
	manualset3
94200	1	400533	13	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of the isoforms , the INM protein Heh2-green fluorescent protein ( GFP ) localized to cytoplasmic membranes , whereas its wild-type localization at the nuclear periphery was restored when the Kap60-44 isoform was reintroduced .
	manualset3
94201	2	400533	13	NULL	NULL	0	NULL	isoforms	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of the isoforms , the INM protein Heh2-green fluorescent protein ( GFP ) localized to cytoplasmic membranes , whereas its wild-type localization at the nuclear periphery was restored when the Kap60-44 isoform was reintroduced .
	manualset3
94216	3	400533	13	NULL	NULL	0	NULL	INM protein Heh2-green fluorescent protein ( GFP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of the isoforms , the INM protein Heh2-green fluorescent protein ( GFP ) localized to cytoplasmic membranes , whereas its wild-type localization at the nuclear periphery was restored when the Kap60-44 isoform was reintroduced .
	manualset3
94217	4	400533	13	NULL	NULL	0	NULL	cytoplasmic membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of the isoforms , the INM protein Heh2-green fluorescent protein ( GFP ) localized to cytoplasmic membranes , whereas its wild-type localization at the nuclear periphery was restored when the Kap60-44 isoform was reintroduced .
	manualset3
94218	5	400533	13	NULL	NULL	0	NULL	wild-type 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of the isoforms , the INM protein Heh2-green fluorescent protein ( GFP ) localized to cytoplasmic membranes , whereas its wild-type localization at the nuclear periphery was restored when the Kap60-44 isoform was reintroduced .
	manualset3
94219	6	400533	13	NULL	NULL	0	NULL	localization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of the isoforms , the INM protein Heh2-green fluorescent protein ( GFP ) localized to cytoplasmic membranes , whereas its wild-type localization at the nuclear periphery was restored when the Kap60-44 isoform was reintroduced .
	manualset3
94220	7	400533	13	NULL	NULL	0	NULL	nuclear periphery	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of the isoforms , the INM protein Heh2-green fluorescent protein ( GFP ) localized to cytoplasmic membranes , whereas its wild-type localization at the nuclear periphery was restored when the Kap60-44 isoform was reintroduced .
	manualset3
94221	8	400533	13	NULL	NULL	0	NULL	Kap60-44 isoform	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of the isoforms , the INM protein Heh2-green fluorescent protein ( GFP ) localized to cytoplasmic membranes , whereas its wild-type localization at the nuclear periphery was restored when the Kap60-44 isoform was reintroduced .
	manualset3
94222	1	400534	13	NULL	NULL	0	NULL	absence of vertical transmission	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of vertical transmission , adverse effects like neonatal seizures , encephalopathy , cerebral palsy , and even neonatal death can still occur .
	manualset3
94223	2	400534	13	NULL	NULL	0	NULL	adverse effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of vertical transmission , adverse effects like neonatal seizures , encephalopathy , cerebral palsy , and even neonatal death can still occur .
	manualset3
94224	3	400534	13	NULL	NULL	0	NULL	neonatal seizures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of vertical transmission , adverse effects like neonatal seizures , encephalopathy , cerebral palsy , and even neonatal death can still occur .
	manualset3
94225	4	400534	13	NULL	NULL	0	NULL	encephalopathy 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of vertical transmission , adverse effects like neonatal seizures , encephalopathy , cerebral palsy , and even neonatal death can still occur .
	manualset3
94226	5	400534	13	NULL	NULL	0	NULL	cerebral palsy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of vertical transmission , adverse effects like neonatal seizures , encephalopathy , cerebral palsy , and even neonatal death can still occur .
	manualset3
94227	6	400534	13	NULL	NULL	0	NULL	neonatal death 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of vertical transmission , adverse effects like neonatal seizures , encephalopathy , cerebral palsy , and even neonatal death can still occur .
	manualset3
94228	1	400535	13	NULL	NULL	0	NULL	active phase	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the active phase of root resorption , the resorption organ contained many odontoclasts with a well-developed ruffled border and a reduced clear zone , cementoblasts , fibroblasts , macrophages , neutrophils , and many blood vessels .
	manualset3
94229	2	400535	13	NULL	NULL	0	NULL	root resorption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the active phase of root resorption , the resorption organ contained many odontoclasts with a well-developed ruffled border and a reduced clear zone , cementoblasts , fibroblasts , macrophages , neutrophils , and many blood vessels .
	manualset3
94230	3	400535	13	NULL	NULL	0	NULL	resorption organ 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the active phase of root resorption , the resorption organ contained many odontoclasts with a well-developed ruffled border and a reduced clear zone , cementoblasts , fibroblasts , macrophages , neutrophils , and many blood vessels .
	manualset3
94231	4	400535	13	NULL	NULL	0	NULL	odontoclasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the active phase of root resorption , the resorption organ contained many odontoclasts with a well-developed ruffled border and a reduced clear zone , cementoblasts , fibroblasts , macrophages , neutrophils , and many blood vessels .
	manualset3
94232	5	400535	13	NULL	NULL	0	NULL	ruffled border	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In the active phase of root resorption , the resorption organ contained many odontoclasts with a well-developed ruffled border and a reduced clear zone , cementoblasts , fibroblasts , macrophages , neutrophils , and many blood vessels .
	manualset3
94233	6	400535	13	NULL	NULL	0	NULL	clear zone	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In the active phase of root resorption , the resorption organ contained many odontoclasts with a well-developed ruffled border and a reduced clear zone , cementoblasts , fibroblasts , macrophages , neutrophils , and many blood vessels .
	manualset3
94234	7	400535	13	NULL	NULL	0	NULL	cementoblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the active phase of root resorption , the resorption organ contained many odontoclasts with a well-developed ruffled border and a reduced clear zone , cementoblasts , fibroblasts , macrophages , neutrophils , and many blood vessels .
	manualset3
94235	8	400535	13	NULL	NULL	0	NULL	fibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the active phase of root resorption , the resorption organ contained many odontoclasts with a well-developed ruffled border and a reduced clear zone , cementoblasts , fibroblasts , macrophages , neutrophils , and many blood vessels .
	manualset3
94236	9	400535	13	NULL	NULL	0	NULL	macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the active phase of root resorption , the resorption organ contained many odontoclasts with a well-developed ruffled border and a reduced clear zone , cementoblasts , fibroblasts , macrophages , neutrophils , and many blood vessels .
	manualset3
94237	10	400535	13	NULL	NULL	0	NULL	neutrophils 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the active phase of root resorption , the resorption organ contained many odontoclasts with a well-developed ruffled border and a reduced clear zone , cementoblasts , fibroblasts , macrophages , neutrophils , and many blood vessels .
	manualset3
94238	11	400535	13	NULL	NULL	0	NULL	blood vessels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the active phase of root resorption , the resorption organ contained many odontoclasts with a well-developed ruffled border and a reduced clear zone , cementoblasts , fibroblasts , macrophages , neutrophils , and many blood vessels .
	manualset3
94239	1	400536	13	NULL	NULL	0	NULL	adrenal medulla	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the adrenal medulla , 6-OHDA did not alter NA concentrations but increased tyrosine hydroxylase activity whereas reserpine depleted noradrenaline and increased tyrosine hydroxylase activity .4 .
	manualset3
94240	2	400536	13	NULL	NULL	0	NULL	6-OHDA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the adrenal medulla , 6-OHDA did not alter NA concentrations but increased tyrosine hydroxylase activity whereas reserpine depleted noradrenaline and increased tyrosine hydroxylase activity .4 .
	manualset3
94241	3	400536	13	NULL	NULL	0	NULL	 NA concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the adrenal medulla , 6-OHDA did not alter NA concentrations but increased tyrosine hydroxylase activity whereas reserpine depleted noradrenaline and increased tyrosine hydroxylase activity .4 .
	manualset3
94242	4	400536	13	NULL	NULL	0	NULL	tyrosine hydroxylase activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the adrenal medulla , 6-OHDA did not alter NA concentrations but increased tyrosine hydroxylase activity whereas reserpine depleted noradrenaline and increased tyrosine hydroxylase activity .4 .
	manualset3
94243	5	400536	13	NULL	NULL	0	NULL	reserpine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the adrenal medulla , 6-OHDA did not alter NA concentrations but increased tyrosine hydroxylase activity whereas reserpine depleted noradrenaline and increased tyrosine hydroxylase activity .4 .
	manualset3
94244	6	400536	13	NULL	NULL	0	NULL	noradrenaline	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the adrenal medulla , 6-OHDA did not alter NA concentrations but increased tyrosine hydroxylase activity whereas reserpine depleted noradrenaline and increased tyrosine hydroxylase activity .4 .
	manualset3
94245	7	400536	13	NULL	NULL	NULL	NULL	tyrosine hydroxylase activity 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the adrenal medulla , 6-OHDA did not alter NA concentrations but increased tyrosine hydroxylase activity whereas reserpine depleted noradrenaline and increased tyrosine hydroxylase activity .4 .
	manualset3
94246	1	400537	13	NULL	NULL	0	NULL	 adult	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In the adult , the liver has the highest levels of Sod1 mRNA and the spleen the highest level of Gpx1 mRNA .
	manualset3
94247	2	400537	13	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the adult , the liver has the highest levels of Sod1 mRNA and the spleen the highest level of Gpx1 mRNA .
	manualset3
94248	3	400537	13	NULL	NULL	0	NULL	 levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the adult , the liver has the highest levels of Sod1 mRNA and the spleen the highest level of Gpx1 mRNA .
	manualset3
94249	4	400537	13	NULL	NULL	0	NULL	Sod1 mRNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the adult , the liver has the highest levels of Sod1 mRNA and the spleen the highest level of Gpx1 mRNA .
	manualset3
94250	5	400537	13	NULL	NULL	0	NULL	spleen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the adult , the liver has the highest levels of Sod1 mRNA and the spleen the highest level of Gpx1 mRNA .
	manualset3
94251	6	400537	13	NULL	NULL	0	NULL	 level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the adult , the liver has the highest levels of Sod1 mRNA and the spleen the highest level of Gpx1 mRNA .
	manualset3
94252	7	400537	13	NULL	NULL	0	NULL	Gpx1 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the adult , the liver has the highest levels of Sod1 mRNA and the spleen the highest level of Gpx1 mRNA .
	manualset3
94253	1	400538	13	NULL	NULL	0	NULL	 adult	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In the adult CNS , however , transplanted neurons and their growing neurites can become confined to the graft region , and there may also be a relative paucity of afferents innervating grafted neurons .
	manualset3
94254	2	400538	13	NULL	NULL	0	NULL	CNS	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the adult CNS , however , transplanted neurons and their growing neurites can become confined to the graft region , and there may also be a relative paucity of afferents innervating grafted neurons .
	manualset3
94255	3	400538	13	NULL	NULL	NULL	NULL	neurons	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the adult CNS , however , transplanted neurons and their growing neurites can become confined to the graft region , and there may also be a relative paucity of afferents innervating grafted neurons .
	manualset3
94256	4	400538	13	NULL	NULL	NULL	NULL	neurites	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the adult CNS , however , transplanted neurons and their growing neurites can become confined to the graft region , and there may also be a relative paucity of afferents innervating grafted neurons .
	manualset3
94257	5	400538	13	NULL	NULL	0	NULL	graft region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the adult CNS , however , transplanted neurons and their growing neurites can become confined to the graft region , and there may also be a relative paucity of afferents innervating grafted neurons .
	manualset3
94258	6	400538	13	NULL	NULL	0	NULL	paucity of afferents	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the adult CNS , however , transplanted neurons and their growing neurites can become confined to the graft region , and there may also be a relative paucity of afferents innervating grafted neurons .
	manualset3
94259	7	400538	13	NULL	NULL	0	NULL	neurons 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the adult CNS , however , transplanted neurons and their growing neurites can become confined to the graft region , and there may also be a relative paucity of afferents innervating grafted neurons .
	manualset3
94260	1	400539	13	NULL	NULL	0	NULL	albino rabbit eyes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the albino rabbit eyes , the chick embryo eyes and the human eye , the concentration of chloride ion in the cytoplasm of retinal pigment epithelium ( RPE ) was high , and in the bullfrog eyes , the concentration was low .
	manualset3
94261	2	400539	13	NULL	NULL	0	NULL	chick embryo eyes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the albino rabbit eyes , the chick embryo eyes and the human eye , the concentration of chloride ion in the cytoplasm of retinal pigment epithelium ( RPE ) was high , and in the bullfrog eyes , the concentration was low .
	manualset3
94262	3	400539	13	NULL	NULL	0	NULL	human eye	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the albino rabbit eyes , the chick embryo eyes and the human eye , the concentration of chloride ion in the cytoplasm of retinal pigment epithelium ( RPE ) was high , and in the bullfrog eyes , the concentration was low .
	manualset3
94263	4	400539	13	NULL	NULL	0	NULL	concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the albino rabbit eyes , the chick embryo eyes and the human eye , the concentration of chloride ion in the cytoplasm of retinal pigment epithelium ( RPE ) was high , and in the bullfrog eyes , the concentration was low .
	manualset3
94264	5	400539	13	NULL	NULL	0	NULL	chloride ion 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In the albino rabbit eyes , the chick embryo eyes and the human eye , the concentration of chloride ion in the cytoplasm of retinal pigment epithelium ( RPE ) was high , and in the bullfrog eyes , the concentration was low .
	manualset3
94265	6	400539	13	NULL	NULL	NULL	NULL	cytoplasm 	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the albino rabbit eyes , the chick embryo eyes and the human eye , the concentration of chloride ion in the cytoplasm of retinal pigment epithelium ( RPE ) was high , and in the bullfrog eyes , the concentration was low .
	manualset3
94266	8	400539	13	NULL	NULL	NULL	NULL	bullfrog eyes	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the albino rabbit eyes , the chick embryo eyes and the human eye , the concentration of chloride ion in the cytoplasm of retinal pigment epithelium ( RPE ) was high , and in the bullfrog eyes , the concentration was low .
	manualset3
94267	9	400539	13	NULL	NULL	NULL	NULL	concentration	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the albino rabbit eyes , the chick embryo eyes and the human eye , the concentration of chloride ion in the cytoplasm of retinal pigment epithelium ( RPE ) was high , and in the bullfrog eyes , the concentration was low .
	manualset3
97109	7	400539	13	NULL	NULL	0	NULL	retinal pigment epithelium ( RPE )	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In the albino rabbit eyes , the chick embryo eyes and the human eye , the concentration of chloride ion in the cytoplasm of retinal pigment epithelium ( RPE ) was high , and in the bullfrog eyes , the concentration was low .
	manualset3
94268	1	400540	13	NULL	NULL	0	NULL	 amphidiploid genome 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the amphidiploid genome of oilseed rape ( Brassica napus ) the diploid ancestral genomes of B. campestris and B. oleracea have been merged .
	manualset3
94269	2	400540	13	NULL	NULL	0	NULL	oilseed rape ( Brassica napus )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the amphidiploid genome of oilseed rape ( Brassica napus ) the diploid ancestral genomes of B. campestris and B. oleracea have been merged .
	manualset3
94270	3	400540	13	NULL	NULL	0	NULL	diploid ancestral genomes 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the amphidiploid genome of oilseed rape ( Brassica napus ) the diploid ancestral genomes of B. campestris and B. oleracea have been merged .
	manualset3
94271	4	400540	13	NULL	NULL	0	NULL	 B. campestris 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the amphidiploid genome of oilseed rape ( Brassica napus ) the diploid ancestral genomes of B. campestris and B. oleracea have been merged .
	manualset3
94272	5	400540	13	NULL	NULL	0	NULL	B. oleracea	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the amphidiploid genome of oilseed rape ( Brassica napus ) the diploid ancestral genomes of B. campestris and B. oleracea have been merged .
	manualset3
94273	1	400541	13	NULL	NULL	0	NULL	1-Methyl-4-phenyl-1 , 2 , 3 , 6 - tetrahydropyridine ( MPTP )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	1-Methyl-4-phenyl-1 , 2 , 3 , 6 - tetrahydropyridine ( MPTP ) - induced neurotoxicity is the most common experimental model used to investigate the pathogenesis of PD .
	manualset3
94274	2	400541	13	NULL	NULL	0	NULL	neurotoxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	1-Methyl-4-phenyl-1 , 2 , 3 , 6 - tetrahydropyridine ( MPTP ) - induced neurotoxicity is the most common experimental model used to investigate the pathogenesis of PD .
	manualset3
94275	3	400541	13	NULL	NULL	NULL	NULL	experimental model	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	1-Methyl-4-phenyl-1 , 2 , 3 , 6 - tetrahydropyridine ( MPTP ) - induced neurotoxicity is the most common experimental model used to investigate the pathogenesis of PD .
	manualset3
94276	4	400541	13	NULL	NULL	0	NULL	pathogenesis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	1-Methyl-4-phenyl-1 , 2 , 3 , 6 - tetrahydropyridine ( MPTP ) - induced neurotoxicity is the most common experimental model used to investigate the pathogenesis of PD .
	manualset3
94277	5	400541	13	NULL	NULL	0	NULL	PD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	1-Methyl-4-phenyl-1 , 2 , 3 , 6 - tetrahydropyridine ( MPTP ) - induced neurotoxicity is the most common experimental model used to investigate the pathogenesis of PD .
	manualset3
94278	1	400542	13	NULL	NULL	0	NULL	anaerobic microflora	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the anaerobic microflora the numbers of clostridia and fusobacteria decreased significantly during the administration period while no other major changes occurred .
	manualset3
94279	2	400542	13	NULL	NULL	0	NULL	 numbers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the anaerobic microflora the numbers of clostridia and fusobacteria decreased significantly during the administration period while no other major changes occurred .
	manualset3
94280	3	400542	13	NULL	NULL	0	NULL	clostridia	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the anaerobic microflora the numbers of clostridia and fusobacteria decreased significantly during the administration period while no other major changes occurred .
	manualset3
94281	4	400542	13	NULL	NULL	0	NULL	fusobacteria 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the anaerobic microflora the numbers of clostridia and fusobacteria decreased significantly during the administration period while no other major changes occurred .
	manualset3
94282	5	400542	13	NULL	NULL	0	NULL	administration period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the anaerobic microflora the numbers of clostridia and fusobacteria decreased significantly during the administration period while no other major changes occurred .
	manualset3
94283	6	400542	13	NULL	NULL	0	NULL	major changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the anaerobic microflora the numbers of clostridia and fusobacteria decreased significantly during the administration period while no other major changes occurred .
	manualset3
94284	1	400543	13	NULL	NULL	0	NULL	anoxic portions	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the anoxic portions of the lake ( 27-34 m ) a net addition of 12C to the DIC pool occurs via organic matter decomposition .
	manualset3
94285	2	400543	13	NULL	NULL	0	NULL	 lake	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the anoxic portions of the lake ( 27-34 m ) a net addition of 12C to the DIC pool occurs via organic matter decomposition .
	manualset3
94286	3	400543	13	NULL	NULL	0	NULL	27-34 m	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the anoxic portions of the lake ( 27-34 m ) a net addition of 12C to the DIC pool occurs via organic matter decomposition .
	manualset3
94287	4	400543	13	NULL	NULL	0	NULL	net addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the anoxic portions of the lake ( 27-34 m ) a net addition of 12C to the DIC pool occurs via organic matter decomposition .
	manualset3
94288	5	400543	13	NULL	NULL	0	NULL	12C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the anoxic portions of the lake ( 27-34 m ) a net addition of 12C to the DIC pool occurs via organic matter decomposition .
	manualset3
94289	6	400543	13	NULL	NULL	0	NULL	DIC pool	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the anoxic portions of the lake ( 27-34 m ) a net addition of 12C to the DIC pool occurs via organic matter decomposition .
	manualset3
94290	7	400543	13	NULL	NULL	0	NULL	organic matter decomposition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the anoxic portions of the lake ( 27-34 m ) a net addition of 12C to the DIC pool occurs via organic matter decomposition .
	manualset3
94291	1	400544	13	NULL	NULL	0	NULL	 arrays results	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the arrays results , the addition of BMP-2 alone led to the expression of genes involved in ( minor ) inflammation .
	manualset3
94292	2	400544	13	NULL	NULL	0	NULL	addition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the arrays results , the addition of BMP-2 alone led to the expression of genes involved in ( minor ) inflammation .
	manualset3
94293	3	400544	13	NULL	NULL	0	NULL	BMP-2 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In the arrays results , the addition of BMP-2 alone led to the expression of genes involved in ( minor ) inflammation .
	manualset3
94294	4	400544	13	NULL	NULL	0	NULL	expression of genes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the arrays results , the addition of BMP-2 alone led to the expression of genes involved in ( minor ) inflammation .
	manualset3
94295	5	400544	13	NULL	NULL	0	NULL	 inflammation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the arrays results , the addition of BMP-2 alone led to the expression of genes involved in ( minor ) inflammation .
	manualset3
94296	1	400545	13	NULL	NULL	0	NULL	 asymmetric 2-methyl benzenethiolate SAM	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the asymmetric 2-methyl benzenethiolate SAM , SFG can simultaneously monitor CH-stretching transitions of both phenyl and methyl groups .
	manualset3
94297	2	400545	13	NULL	NULL	0	NULL	SFG 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the asymmetric 2-methyl benzenethiolate SAM , SFG can simultaneously monitor CH-stretching transitions of both phenyl and methyl groups .
	manualset3
94298	3	400545	13	NULL	NULL	0	NULL	monitor 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the asymmetric 2-methyl benzenethiolate SAM , SFG can simultaneously monitor CH-stretching transitions of both phenyl and methyl groups .
	manualset3
94299	4	400545	13	NULL	NULL	NULL	NULL	CH-stretching transitions of phenyl  groups	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the asymmetric 2-methyl benzenethiolate SAM , SFG can simultaneously monitor CH-stretching transitions of both phenyl and methyl groups .
	manualset3
97110	5	400545	13	NULL	NULL	0	NULL	CH-stretching transitions of methyl groups	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the asymmetric 2-methyl benzenethiolate SAM , SFG can simultaneously monitor CH-stretching transitions of both phenyl and methyl groups .
	manualset3
94300	1	400546	13	NULL	NULL	0	NULL	battery manufacturing plant 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In the battery manufacturing plant , full-shift area samples taken across 5 days in several production areas showed a mean value SD of 349 107 g/m ( 3 ) , while area samples in the office area had a mean SD of 55.2 33.2 g/m ( 3 ) .
	manualset3
94301	2	400546	13	NULL	NULL	NULL	NULL	full-shift area samples	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the battery manufacturing plant , full-shift area samples taken across 5 days in several production areas showed a mean value SD of 349 107 g/m ( 3 ) , while area samples in the office area had a mean SD of 55.2 33.2 g/m ( 3 ) .
	manualset3
94302	3	400546	13	NULL	NULL	NULL	NULL	 5 days 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the battery manufacturing plant , full-shift area samples taken across 5 days in several production areas showed a mean value SD of 349 107 g/m ( 3 ) , while area samples in the office area had a mean SD of 55.2 33.2 g/m ( 3 ) .
	manualset3
94303	4	400546	13	NULL	NULL	0	NULL	 several production areas	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the battery manufacturing plant , full-shift area samples taken across 5 days in several production areas showed a mean value SD of 349 107 g/m ( 3 ) , while area samples in the office area had a mean SD of 55.2 33.2 g/m ( 3 ) .
	manualset3
94304	5	400546	13	NULL	NULL	0	NULL	 mean value SD of 349 107 g/m ( 3 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the battery manufacturing plant , full-shift area samples taken across 5 days in several production areas showed a mean value SD of 349 107 g/m ( 3 ) , while area samples in the office area had a mean SD of 55.2 33.2 g/m ( 3 ) .
	manualset3
94305	6	400546	13	NULL	NULL	NULL	NULL	area samples	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the battery manufacturing plant , full-shift area samples taken across 5 days in several production areas showed a mean value SD of 349 107 g/m ( 3 ) , while area samples in the office area had a mean SD of 55.2 33.2 g/m ( 3 ) .
	manualset3
94306	7	400546	13	NULL	NULL	0	NULL	office area	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the battery manufacturing plant , full-shift area samples taken across 5 days in several production areas showed a mean value SD of 349 107 g/m ( 3 ) , while area samples in the office area had a mean SD of 55.2 33.2 g/m ( 3 ) .
	manualset3
94307	8	400546	13	NULL	NULL	0	NULL	mean SD of 55.2 33.2 g/m ( 3 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the battery manufacturing plant , full-shift area samples taken across 5 days in several production areas showed a mean value SD of 349 107 g/m ( 3 ) , while area samples in the office area had a mean SD of 55.2 33.2 g/m ( 3 ) .
	manualset3
94308	1	400547	13	NULL	NULL	NULL	NULL	beta subunit , P136G	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the beta and gamma subunits , P136G prevented assembly of higher order heteroligomers , whereas in the alpha and delta subunits , P136G prevented transport of assembled pentamers to the cell surface .
	manualset3
94309	2	400547	13	NULL	NULL	0	NULL	assembly of higher order heteroligomers 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the beta and gamma subunits , P136G prevented assembly of higher order heteroligomers , whereas in the alpha and delta subunits , P136G prevented transport of assembled pentamers to the cell surface .
	manualset3
94310	3	400547	13	NULL	NULL	NULL	NULL	alpha subunit, P136G	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the beta and gamma subunits , P136G prevented assembly of higher order heteroligomers , whereas in the alpha and delta subunits , P136G prevented transport of assembled pentamers to the cell surface .
	manualset3
94311	4	400547	13	NULL	NULL	0	NULL	transport of assembled pentamers	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the beta and gamma subunits , P136G prevented assembly of higher order heteroligomers , whereas in the alpha and delta subunits , P136G prevented transport of assembled pentamers to the cell surface .
	manualset3
94312	5	400547	13	NULL	NULL	0	NULL	cell surface	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In the beta and gamma subunits , P136G prevented assembly of higher order heteroligomers , whereas in the alpha and delta subunits , P136G prevented transport of assembled pentamers to the cell surface .
	manualset3
98576	6	400547	13	NULL	NULL	0	NULL	gamma subunit, P136G	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the beta and gamma subunits , P136G prevented assembly of higher order heteroligomers , whereas in the alpha and delta subunits , P136G prevented transport of assembled pentamers to the cell surface .
	manualset3
98577	7	400547	13	NULL	NULL	0	NULL	delta subunit, P136G	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the beta and gamma subunits , P136G prevented assembly of higher order heteroligomers , whereas in the alpha and delta subunits , P136G prevented transport of assembled pentamers to the cell surface .
	manualset3
94313	1	400548	13	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the brain , these receptors are expressed on glial cells , and some recent data have suggested that anaphylatoxins could mediate neuroprotection .
	manualset3
94314	2	400548	13	NULL	NULL	0	NULL	receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the brain , these receptors are expressed on glial cells , and some recent data have suggested that anaphylatoxins could mediate neuroprotection .
	manualset3
94315	3	400548	13	NULL	NULL	0	NULL	glial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the brain , these receptors are expressed on glial cells , and some recent data have suggested that anaphylatoxins could mediate neuroprotection .
	manualset3
94316	4	400548	13	NULL	NULL	0	NULL	recent data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the brain , these receptors are expressed on glial cells , and some recent data have suggested that anaphylatoxins could mediate neuroprotection .
	manualset3
94317	5	400548	13	NULL	NULL	0	NULL	 anaphylatoxins	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	In the brain , these receptors are expressed on glial cells , and some recent data have suggested that anaphylatoxins could mediate neuroprotection .
	manualset3
94319	6	400548	13	NULL	NULL	0	NULL	neuroprotection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the brain , these receptors are expressed on glial cells , and some recent data have suggested that anaphylatoxins could mediate neuroprotection .
	manualset3
94320	1	400549	13	NULL	NULL	0	NULL	breakfast experiment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the breakfast experiment , seven young adult subjects ingested a meal containing 291 microgram of retinol equivalents .
	manualset3
94321	2	400549	13	NULL	NULL	0	NULL	seven 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the breakfast experiment , seven young adult subjects ingested a meal containing 291 microgram of retinol equivalents .
	manualset3
94322	3	400549	13	NULL	NULL	0	NULL	young adult subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the breakfast experiment , seven young adult subjects ingested a meal containing 291 microgram of retinol equivalents .
	manualset3
94323	4	400549	13	NULL	NULL	0	NULL	meal 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	In the breakfast experiment , seven young adult subjects ingested a meal containing 291 microgram of retinol equivalents .
	manualset3
94324	5	400549	13	NULL	NULL	0	NULL	291 microgram	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the breakfast experiment , seven young adult subjects ingested a meal containing 291 microgram of retinol equivalents .
	manualset3
94325	6	400549	13	NULL	NULL	0	NULL	retinol equivalents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the breakfast experiment , seven young adult subjects ingested a meal containing 291 microgram of retinol equivalents .
	manualset3
94326	1	400550	13	NULL	NULL	0	NULL	budding yeast Saccharomyces cerevisiae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the budding yeast Saccharomyces cerevisiae , centrosomal functions are provided by the spindle pole body ( SPB ) , which is duplicated at the time of bud emergence in G1 of the cell cycle .
	manualset3
94327	2	400550	13	NULL	NULL	0	NULL	centrosomal functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the budding yeast Saccharomyces cerevisiae , centrosomal functions are provided by the spindle pole body ( SPB ) , which is duplicated at the time of bud emergence in G1 of the cell cycle .
	manualset3
94328	3	400550	13	NULL	NULL	NULL	NULL	spindle pole body ( SPB )	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the budding yeast Saccharomyces cerevisiae , centrosomal functions are provided by the spindle pole body ( SPB ) , which is duplicated at the time of bud emergence in G1 of the cell cycle .
	manualset3
94329	4	400550	13	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In the budding yeast Saccharomyces cerevisiae , centrosomal functions are provided by the spindle pole body ( SPB ) , which is duplicated at the time of bud emergence in G1 of the cell cycle .
	manualset3
94330	5	400550	13	NULL	NULL	0	NULL	bud emergence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the budding yeast Saccharomyces cerevisiae , centrosomal functions are provided by the spindle pole body ( SPB ) , which is duplicated at the time of bud emergence in G1 of the cell cycle .
	manualset3
94331	6	400550	13	NULL	NULL	NULL	NULL	G1 of the cell cycle	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the budding yeast Saccharomyces cerevisiae , centrosomal functions are provided by the spindle pole body ( SPB ) , which is duplicated at the time of bud emergence in G1 of the cell cycle .
	manualset3
94332	1	400551	13	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	1.21 ) is the first committed enzyme of the sterol biosynthesis pathway .
	manualset3
94333	2	400551	13	NULL	NULL	0	NULL	 sterol biosynthesis pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	1.21 ) is the first committed enzyme of the sterol biosynthesis pathway .
	manualset3
94334	1	400552	13	NULL	NULL	0	NULL	case	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case being reported on here of a lady patient aged 64 and suffering from a toxic adenoma not recognized at the time , thyrotoxicosis accompanied by above-normal FT-3 results and the characteristic clinical symptoms developed when lithium medication was discontinued .
	manualset3
94335	2	400552	13	NULL	NULL	0	NULL	lady patient aged 64	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case being reported on here of a lady patient aged 64 and suffering from a toxic adenoma not recognized at the time , thyrotoxicosis accompanied by above-normal FT-3 results and the characteristic clinical symptoms developed when lithium medication was discontinued .
	manualset3
94337	4	400552	13	NULL	NULL	0	NULL	toxic adenoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case being reported on here of a lady patient aged 64 and suffering from a toxic adenoma not recognized at the time , thyrotoxicosis accompanied by above-normal FT-3 results and the characteristic clinical symptoms developed when lithium medication was discontinued .
	manualset3
94338	5	400552	13	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case being reported on here of a lady patient aged 64 and suffering from a toxic adenoma not recognized at the time , thyrotoxicosis accompanied by above-normal FT-3 results and the characteristic clinical symptoms developed when lithium medication was discontinued .
	manualset3
94339	6	400552	13	NULL	NULL	0	NULL	 thyrotoxicosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case being reported on here of a lady patient aged 64 and suffering from a toxic adenoma not recognized at the time , thyrotoxicosis accompanied by above-normal FT-3 results and the characteristic clinical symptoms developed when lithium medication was discontinued .
	manualset3
94340	7	400552	13	NULL	NULL	NULL	NULL	FT-3 results 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the case being reported on here of a lady patient aged 64 and suffering from a toxic adenoma not recognized at the time , thyrotoxicosis accompanied by above-normal FT-3 results and the characteristic clinical symptoms developed when lithium medication was discontinued .
	manualset3
94341	8	400552	13	NULL	NULL	NULL	NULL	clinical symptoms	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the case being reported on here of a lady patient aged 64 and suffering from a toxic adenoma not recognized at the time , thyrotoxicosis accompanied by above-normal FT-3 results and the characteristic clinical symptoms developed when lithium medication was discontinued .
	manualset3
94342	9	400552	13	NULL	NULL	0	NULL	lithium medication	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case being reported on here of a lady patient aged 64 and suffering from a toxic adenoma not recognized at the time , thyrotoxicosis accompanied by above-normal FT-3 results and the characteristic clinical symptoms developed when lithium medication was discontinued .
	manualset3
94343	1	400553	13	NULL	NULL	0	NULL	case	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of Actinomyces olivaceus , phosphatidyl ethanolamine and ornithine containing a phosphorus-lacking lipid can be regarded , this being corroborated by comparative data about their quantitative content .
	manualset3
94344	2	400553	13	NULL	NULL	0	NULL	Actinomyces olivaceus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of Actinomyces olivaceus , phosphatidyl ethanolamine and ornithine containing a phosphorus-lacking lipid can be regarded , this being corroborated by comparative data about their quantitative content .
	manualset3
94345	3	400553	13	NULL	NULL	0	NULL	phosphatidyl ethanolamine 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of Actinomyces olivaceus , phosphatidyl ethanolamine and ornithine containing a phosphorus-lacking lipid can be regarded , this being corroborated by comparative data about their quantitative content .
	manualset3
94346	4	400553	13	NULL	NULL	0	NULL	ornithine containing a phosphorus-lacking lipid 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of Actinomyces olivaceus , phosphatidyl ethanolamine and ornithine containing a phosphorus-lacking lipid can be regarded , this being corroborated by comparative data about their quantitative content .
	manualset3
94347	5	400553	13	NULL	NULL	0	NULL	comparative data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of Actinomyces olivaceus , phosphatidyl ethanolamine and ornithine containing a phosphorus-lacking lipid can be regarded , this being corroborated by comparative data about their quantitative content .
	manualset3
94348	6	400553	13	NULL	NULL	0	NULL	quantitative content 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of Actinomyces olivaceus , phosphatidyl ethanolamine and ornithine containing a phosphorus-lacking lipid can be regarded , this being corroborated by comparative data about their quantitative content .
	manualset3
94349	1	400554	13	NULL	NULL	0	NULL	case of FIV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of FIV , males were twice as likely to be infected as females , and cats over 10 years of age were 13.5 times more likely to be infected than cats less than 1 year of age .
	manualset3
94350	2	400554	13	NULL	NULL	NULL	NULL	males 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the case of FIV , males were twice as likely to be infected as females , and cats over 10 years of age were 13.5 times more likely to be infected than cats less than 1 year of age .
	manualset3
94351	3	400554	13	NULL	NULL	NULL	NULL	females	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the case of FIV , males were twice as likely to be infected as females , and cats over 10 years of age were 13.5 times more likely to be infected than cats less than 1 year of age .
	manualset3
94352	4	400554	13	NULL	NULL	0	NULL	 cats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of FIV , males were twice as likely to be infected as females , and cats over 10 years of age were 13.5 times more likely to be infected than cats less than 1 year of age .
	manualset3
94353	5	400554	13	NULL	NULL	0	NULL	10 years of age	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of FIV , males were twice as likely to be infected as females , and cats over 10 years of age were 13.5 times more likely to be infected than cats less than 1 year of age .
	manualset3
94354	6	400554	13	NULL	NULL	0	NULL	13.5 times	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of FIV , males were twice as likely to be infected as females , and cats over 10 years of age were 13.5 times more likely to be infected than cats less than 1 year of age .
	manualset3
94355	7	400554	13	NULL	NULL	0	NULL	cats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of FIV , males were twice as likely to be infected as females , and cats over 10 years of age were 13.5 times more likely to be infected than cats less than 1 year of age .
	manualset3
94356	8	400554	13	NULL	NULL	0	NULL	1 year of age 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of FIV , males were twice as likely to be infected as females , and cats over 10 years of age were 13.5 times more likely to be infected than cats less than 1 year of age .
	manualset3
94357	1	400555	13	NULL	NULL	NULL	NULL	aFGF	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the case of aFGF , suramin interacts at or near its heparin binding site .
	manualset3
94358	2	400555	13	NULL	NULL	0	NULL	suramin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of aFGF , suramin interacts at or near its heparin binding site .
	manualset3
94359	3	400555	13	NULL	NULL	0	NULL	heparin binding site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of aFGF , suramin interacts at or near its heparin binding site .
	manualset3
98578	4	400555	13	NULL	NULL	0	NULL	case	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of aFGF , suramin interacts at or near its heparin binding site .
	manualset3
94360	1	400556	13	NULL	NULL	NULL	NULL	case	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the case of atypical symptoms such as dysphagia , laryngitis , asthma and chest pain , there is more reason to pursue diagnostic testing .
	manualset3
94361	2	400556	13	NULL	NULL	0	NULL	atypical symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of atypical symptoms such as dysphagia , laryngitis , asthma and chest pain , there is more reason to pursue diagnostic testing .
	manualset3
94362	3	400556	13	NULL	NULL	0	NULL	dysphagia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of atypical symptoms such as dysphagia , laryngitis , asthma and chest pain , there is more reason to pursue diagnostic testing .
	manualset3
94363	4	400556	13	NULL	NULL	0	NULL	 laryngitis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of atypical symptoms such as dysphagia , laryngitis , asthma and chest pain , there is more reason to pursue diagnostic testing .
	manualset3
94364	5	400556	13	NULL	NULL	0	NULL	asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of atypical symptoms such as dysphagia , laryngitis , asthma and chest pain , there is more reason to pursue diagnostic testing .
	manualset3
94365	6	400556	13	NULL	NULL	0	NULL	chest pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of atypical symptoms such as dysphagia , laryngitis , asthma and chest pain , there is more reason to pursue diagnostic testing .
	manualset3
94366	7	400556	13	NULL	NULL	0	NULL	reason 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of atypical symptoms such as dysphagia , laryngitis , asthma and chest pain , there is more reason to pursue diagnostic testing .
	manualset3
94367	8	400556	13	NULL	NULL	0	NULL	diagnostic testing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of atypical symptoms such as dysphagia , laryngitis , asthma and chest pain , there is more reason to pursue diagnostic testing .
	manualset3
94368	1	400557	13	NULL	NULL	0	NULL	case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of clinical symptoms such as dysphagia , foreign-body sensation and chronic neck or facial pain close to the ear , an Eagle syndrome should be considered in the differential diagnosis .
	manualset3
94369	2	400557	13	NULL	NULL	0	NULL	clinical symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of clinical symptoms such as dysphagia , foreign-body sensation and chronic neck or facial pain close to the ear , an Eagle syndrome should be considered in the differential diagnosis .
	manualset3
94370	3	400557	13	NULL	NULL	0	NULL	dysphagia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of clinical symptoms such as dysphagia , foreign-body sensation and chronic neck or facial pain close to the ear , an Eagle syndrome should be considered in the differential diagnosis .
	manualset3
94371	4	400557	13	NULL	NULL	0	NULL	foreign-body sensation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of clinical symptoms such as dysphagia , foreign-body sensation and chronic neck or facial pain close to the ear , an Eagle syndrome should be considered in the differential diagnosis .
	manualset3
94372	5	400557	13	NULL	NULL	0	NULL	chronic neck pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of clinical symptoms such as dysphagia , foreign-body sensation and chronic neck or facial pain close to the ear , an Eagle syndrome should be considered in the differential diagnosis .
	manualset3
94373	6	400557	13	NULL	NULL	0	NULL	 facial pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of clinical symptoms such as dysphagia , foreign-body sensation and chronic neck or facial pain close to the ear , an Eagle syndrome should be considered in the differential diagnosis .
	manualset3
94374	7	400557	13	NULL	NULL	0	NULL	 ear	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of clinical symptoms such as dysphagia , foreign-body sensation and chronic neck or facial pain close to the ear , an Eagle syndrome should be considered in the differential diagnosis .
	manualset3
94375	8	400557	13	NULL	NULL	0	NULL	Eagle syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of clinical symptoms such as dysphagia , foreign-body sensation and chronic neck or facial pain close to the ear , an Eagle syndrome should be considered in the differential diagnosis .
	manualset3
94376	9	400557	13	NULL	NULL	0	NULL	differential diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of clinical symptoms such as dysphagia , foreign-body sensation and chronic neck or facial pain close to the ear , an Eagle syndrome should be considered in the differential diagnosis .
	manualset3
94377	1	400558	13	NULL	NULL	NULL	NULL	intratumoral gene transfer	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the case of intratumoral gene transfer , foreign DNA was detected in only one of seven mice by polymerase chain reaction ( PCR ) analysis performed 7 days following injection .
	manualset3
94378	2	400558	13	NULL	NULL	0	NULL	 foreign DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of intratumoral gene transfer , foreign DNA was detected in only one of seven mice by polymerase chain reaction ( PCR ) analysis performed 7 days following injection .
	manualset3
94379	3	400558	13	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of intratumoral gene transfer , foreign DNA was detected in only one of seven mice by polymerase chain reaction ( PCR ) analysis performed 7 days following injection .
	manualset3
94380	4	400558	13	NULL	NULL	0	NULL	seven	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of intratumoral gene transfer , foreign DNA was detected in only one of seven mice by polymerase chain reaction ( PCR ) analysis performed 7 days following injection .
	manualset3
94381	5	400558	13	NULL	NULL	0	NULL	mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of intratumoral gene transfer , foreign DNA was detected in only one of seven mice by polymerase chain reaction ( PCR ) analysis performed 7 days following injection .
	manualset3
94382	6	400558	13	NULL	NULL	0	NULL	polymerase chain reaction ( PCR ) analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of intratumoral gene transfer , foreign DNA was detected in only one of seven mice by polymerase chain reaction ( PCR ) analysis performed 7 days following injection .
	manualset3
94383	7	400558	13	NULL	NULL	NULL	NULL	7 days	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the case of intratumoral gene transfer , foreign DNA was detected in only one of seven mice by polymerase chain reaction ( PCR ) analysis performed 7 days following injection .
	manualset3
94384	8	400558	13	NULL	NULL	0	NULL	injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of intratumoral gene transfer , foreign DNA was detected in only one of seven mice by polymerase chain reaction ( PCR ) analysis performed 7 days following injection .
	manualset3
98579	9	400558	13	NULL	NULL	0	NULL	case	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of intratumoral gene transfer , foreign DNA was detected in only one of seven mice by polymerase chain reaction ( PCR ) analysis performed 7 days following injection .
	manualset3
94385	1	400559	13	NULL	NULL	0	NULL	case	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of rat brain the non-tyrosinatable tubulin pool accounts for about 50 % of the tubulin .
	manualset3
94386	2	400559	13	NULL	NULL	0	NULL	rat brain 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of rat brain the non-tyrosinatable tubulin pool accounts for about 50 % of the tubulin .
	manualset3
94387	3	400559	13	NULL	NULL	0	NULL	non-tyrosinatable tubulin pool	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of rat brain the non-tyrosinatable tubulin pool accounts for about 50 % of the tubulin .
	manualset3
94388	4	400559	13	NULL	NULL	0	NULL	50 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of rat brain the non-tyrosinatable tubulin pool accounts for about 50 % of the tubulin .
	manualset3
94389	5	400559	13	NULL	NULL	0	NULL	tubulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of rat brain the non-tyrosinatable tubulin pool accounts for about 50 % of the tubulin .
	manualset3
94390	1	400560	13	NULL	NULL	NULL	NULL	case	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the case of streptavidin the angular range of the observed diffraction corresponds to a resolution of 10 A in plane and 14 A normal to the plane .
	manualset3
94391	2	400560	13	NULL	NULL	0	NULL	streptavidin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of streptavidin the angular range of the observed diffraction corresponds to a resolution of 10 A in plane and 14 A normal to the plane .
	manualset3
94392	3	400560	13	NULL	NULL	0	NULL	angular range	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of streptavidin the angular range of the observed diffraction corresponds to a resolution of 10 A in plane and 14 A normal to the plane .
	manualset3
94393	4	400560	13	NULL	NULL	0	NULL	diffraction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of streptavidin the angular range of the observed diffraction corresponds to a resolution of 10 A in plane and 14 A normal to the plane .
	manualset3
94394	5	400560	13	NULL	NULL	0	NULL	resolution	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of streptavidin the angular range of the observed diffraction corresponds to a resolution of 10 A in plane and 14 A normal to the plane .
	manualset3
94395	6	400560	13	NULL	NULL	0	NULL	10 A in plane	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of streptavidin the angular range of the observed diffraction corresponds to a resolution of 10 A in plane and 14 A normal to the plane .
	manualset3
94396	7	400560	13	NULL	NULL	0	NULL	14 A normal to the plane	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of streptavidin the angular range of the observed diffraction corresponds to a resolution of 10 A in plane and 14 A normal to the plane .
	manualset3
94397	1	400561	13	NULL	NULL	0	NULL	1.4 mol dm ( -3 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	1.4 mol dm ( -3 ) , probably ion-paired by hydrogen bonds to the chloride ions .
	manualset3
94398	2	400561	13	NULL	NULL	0	NULL	hydrogen bonds	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	1.4 mol dm ( -3 ) , probably ion-paired by hydrogen bonds to the chloride ions .
	manualset3
94399	3	400561	13	NULL	NULL	0	NULL	 chloride ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	1.4 mol dm ( -3 ) , probably ion-paired by hydrogen bonds to the chloride ions .
	manualset3
94400	1	400562	13	NULL	NULL	0	NULL	case	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of the DEB skin equivalent , the newly expressed type VII collagen reversed the DEB phenotype characterized by poor epidermal-dermal adherence and anchoring fibril defects .
	manualset3
94401	2	400562	13	NULL	NULL	0	NULL	DEB skin equivalent	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of the DEB skin equivalent , the newly expressed type VII collagen reversed the DEB phenotype characterized by poor epidermal-dermal adherence and anchoring fibril defects .
	manualset3
94402	3	400562	13	NULL	NULL	0	NULL	type VII collagen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of the DEB skin equivalent , the newly expressed type VII collagen reversed the DEB phenotype characterized by poor epidermal-dermal adherence and anchoring fibril defects .
	manualset3
94403	4	400562	13	NULL	NULL	0	NULL	DEB phenotype	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of the DEB skin equivalent , the newly expressed type VII collagen reversed the DEB phenotype characterized by poor epidermal-dermal adherence and anchoring fibril defects .
	manualset3
94404	5	400562	13	NULL	NULL	0	NULL	poor epidermal-dermal adherence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of the DEB skin equivalent , the newly expressed type VII collagen reversed the DEB phenotype characterized by poor epidermal-dermal adherence and anchoring fibril defects .
	manualset3
94405	6	400562	13	NULL	NULL	NULL	NULL	fibril defects 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the case of the DEB skin equivalent , the newly expressed type VII collagen reversed the DEB phenotype characterized by poor epidermal-dermal adherence and anchoring fibril defects .
	manualset3
94406	1	400563	13	NULL	NULL	0	NULL	case of the plane	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of the plane all of the counter-ions are condensed in the above sense , not just a fraction , for any surface charge density of the plane .
	manualset3
94407	2	400563	13	NULL	NULL	0	NULL	counter-ions 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of the plane all of the counter-ions are condensed in the above sense , not just a fraction , for any surface charge density of the plane .
	manualset3
94408	3	400563	13	NULL	NULL	0	NULL	sense	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of the plane all of the counter-ions are condensed in the above sense , not just a fraction , for any surface charge density of the plane .
	manualset3
94409	4	400563	13	NULL	NULL	0	NULL	 fraction 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of the plane all of the counter-ions are condensed in the above sense , not just a fraction , for any surface charge density of the plane .
	manualset3
94410	5	400563	13	NULL	NULL	0	NULL	surface charge density	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of the plane all of the counter-ions are condensed in the above sense , not just a fraction , for any surface charge density of the plane .
	manualset3
94411	6	400563	13	NULL	NULL	0	NULL	plane	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of the plane all of the counter-ions are condensed in the above sense , not just a fraction , for any surface charge density of the plane .
	manualset3
94412	1	400564	13	NULL	NULL	0	NULL	cases of strong defects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cases of strong defects of morphogenesis in the fi/fi + / + and , especially , fi/fi or/or , embryos gamma-crystallins were not detected .
	manualset3
94413	2	400564	13	NULL	NULL	0	NULL	morphogenesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cases of strong defects of morphogenesis in the fi/fi + / + and , especially , fi/fi or/or , embryos gamma-crystallins were not detected .
	manualset3
94414	3	400564	13	NULL	NULL	NULL	NULL	fi/fi + / +, embryos	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the cases of strong defects of morphogenesis in the fi/fi + / + and , especially , fi/fi or/or , embryos gamma-crystallins were not detected .
	manualset3
94415	4	400564	13	NULL	NULL	0	NULL	fi/fi or/or , embryos	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cases of strong defects of morphogenesis in the fi/fi + / + and , especially , fi/fi or/or , embryos gamma-crystallins were not detected .
	manualset3
94416	5	400564	13	NULL	NULL	0	NULL	gamma-crystallins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cases of strong defects of morphogenesis in the fi/fi + / + and , especially , fi/fi or/or , embryos gamma-crystallins were not detected .
	manualset3
94417	1	400565	13	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cases studied here , with an increasing number of actions , cooperation is increasingly likely to become advantageous compared with pure self-interest , but self-interest can achieve all that cooperation could achieve in a nonnegligible fraction of cases .
	manualset3
94418	2	400565	13	NULL	NULL	0	NULL	number of actions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cases studied here , with an increasing number of actions , cooperation is increasingly likely to become advantageous compared with pure self-interest , but self-interest can achieve all that cooperation could achieve in a nonnegligible fraction of cases .
	manualset3
94419	3	400565	13	NULL	NULL	0	NULL	cooperation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cases studied here , with an increasing number of actions , cooperation is increasingly likely to become advantageous compared with pure self-interest , but self-interest can achieve all that cooperation could achieve in a nonnegligible fraction of cases .
	manualset3
94420	4	400565	13	NULL	NULL	0	NULL	self-interest	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cases studied here , with an increasing number of actions , cooperation is increasingly likely to become advantageous compared with pure self-interest , but self-interest can achieve all that cooperation could achieve in a nonnegligible fraction of cases .
	manualset3
94421	5	400565	13	NULL	NULL	0	NULL	self-interest 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cases studied here , with an increasing number of actions , cooperation is increasingly likely to become advantageous compared with pure self-interest , but self-interest can achieve all that cooperation could achieve in a nonnegligible fraction of cases .
	manualset3
94422	6	400565	13	NULL	NULL	0	NULL	cooperation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cases studied here , with an increasing number of actions , cooperation is increasingly likely to become advantageous compared with pure self-interest , but self-interest can achieve all that cooperation could achieve in a nonnegligible fraction of cases .
	manualset3
94423	7	400565	13	NULL	NULL	0	NULL	nonnegligible fraction of cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cases studied here , with an increasing number of actions , cooperation is increasingly likely to become advantageous compared with pure self-interest , but self-interest can achieve all that cooperation could achieve in a nonnegligible fraction of cases .
	manualset3
94424	1	400566	13	NULL	NULL	0	NULL	cerebellum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cerebellum , the IRK1 protein was clearly detected in the somata and proximal dendrites of Purkinje cells , while the GIRK1 protein was present in the somata and clustered dendrites of granule cells .
	manualset3
94425	2	400566	13	NULL	NULL	0	NULL	IRK1 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cerebellum , the IRK1 protein was clearly detected in the somata and proximal dendrites of Purkinje cells , while the GIRK1 protein was present in the somata and clustered dendrites of granule cells .
	manualset3
94426	3	400566	13	NULL	NULL	0	NULL	somata of Purkinje cells	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cerebellum , the IRK1 protein was clearly detected in the somata and proximal dendrites of Purkinje cells , while the GIRK1 protein was present in the somata and clustered dendrites of granule cells .
	manualset3
94427	4	400566	13	NULL	NULL	0	NULL	proximal dendrites of Purkinje cells	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cerebellum , the IRK1 protein was clearly detected in the somata and proximal dendrites of Purkinje cells , while the GIRK1 protein was present in the somata and clustered dendrites of granule cells .
	manualset3
94428	5	400566	13	NULL	NULL	0	NULL	GIRK1 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cerebellum , the IRK1 protein was clearly detected in the somata and proximal dendrites of Purkinje cells , while the GIRK1 protein was present in the somata and clustered dendrites of granule cells .
	manualset3
94429	6	400566	13	NULL	NULL	0	NULL	somata of granule cells	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cerebellum , the IRK1 protein was clearly detected in the somata and proximal dendrites of Purkinje cells , while the GIRK1 protein was present in the somata and clustered dendrites of granule cells .
	manualset3
94430	7	400566	13	NULL	NULL	0	NULL	clustered dendrites of granule cells 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cerebellum , the IRK1 protein was clearly detected in the somata and proximal dendrites of Purkinje cells , while the GIRK1 protein was present in the somata and clustered dendrites of granule cells .
	manualset3
94431	1	400567	13	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the chronically treated animals , FK506 levels were within the clinically relevant range .
	manualset3
94432	2	400567	13	NULL	NULL	0	NULL	FK506 levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the chronically treated animals , FK506 levels were within the clinically relevant range .
	manualset3
94435	3	400567	13	NULL	NULL	0	NULL	range	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the chronically treated animals , FK506 levels were within the clinically relevant range .
	manualset3
94438	1	400568	13	NULL	NULL	0	NULL	cold ( 10 degrees C ) test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cold ( 10 degrees C ) test , ( + ) - HA966 reversed the ineffectiveness of the highest dose of morphine .
	manualset3
94440	2	400568	13	NULL	NULL	0	NULL	 ( + ) - HA966 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cold ( 10 degrees C ) test , ( + ) - HA966 reversed the ineffectiveness of the highest dose of morphine .
	manualset3
94444	3	400568	13	NULL	NULL	0	NULL	ineffectiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cold ( 10 degrees C ) test , ( + ) - HA966 reversed the ineffectiveness of the highest dose of morphine .
	manualset3
94445	4	400568	13	NULL	NULL	0	NULL	dose of morphine	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cold ( 10 degrees C ) test , ( + ) - HA966 reversed the ineffectiveness of the highest dose of morphine .
	manualset3
94448	1	400569	13	NULL	NULL	0	NULL	analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the combined analyses , a significant association was found between rs8050136 , located in the first intron of the fat mass and obesity-associated ( FTO ) gene , and BMI ( P = 4.97 10 ( -7 ) ) and FFMI ( P = 1.19 10 ( -7 ) ) .
	manualset3
94449	2	400569	13	NULL	NULL	NULL	NULL	association	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the combined analyses , a significant association was found between rs8050136 , located in the first intron of the fat mass and obesity-associated ( FTO ) gene , and BMI ( P = 4.97 10 ( -7 ) ) and FFMI ( P = 1.19 10 ( -7 ) ) .
	manualset3
94450	3	400569	13	NULL	NULL	0	NULL	rs8050136	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the combined analyses , a significant association was found between rs8050136 , located in the first intron of the fat mass and obesity-associated ( FTO ) gene , and BMI ( P = 4.97 10 ( -7 ) ) and FFMI ( P = 1.19 10 ( -7 ) ) .
	manualset3
94451	4	400569	13	NULL	NULL	0	NULL	first intron of the fat mass and obesity-associated ( FTO ) gene	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the combined analyses , a significant association was found between rs8050136 , located in the first intron of the fat mass and obesity-associated ( FTO ) gene , and BMI ( P = 4.97 10 ( -7 ) ) and FFMI ( P = 1.19 10 ( -7 ) ) .
	manualset3
94452	5	400569	13	NULL	NULL	0	NULL	BMI ( P = 4.97 10 ( -7 ) ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the combined analyses , a significant association was found between rs8050136 , located in the first intron of the fat mass and obesity-associated ( FTO ) gene , and BMI ( P = 4.97 10 ( -7 ) ) and FFMI ( P = 1.19 10 ( -7 ) ) .
	manualset3
94453	6	400569	13	NULL	NULL	0	NULL	FFMI ( P = 1.19 10 ( -7 ) )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the combined analyses , a significant association was found between rs8050136 , located in the first intron of the fat mass and obesity-associated ( FTO ) gene , and BMI ( P = 4.97 10 ( -7 ) ) and FFMI ( P = 1.19 10 ( -7 ) ) .
	manualset3
94456	1	400570	13	NULL	NULL	0	NULL	complex eigenvalue approach	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In the complex eigenvalue approach , only linearised equilibrium is analyzed and non-linear behavior of the brake system is not taken into account .
	manualset3
94457	2	400570	13	NULL	NULL	0	NULL	equilibrium	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the complex eigenvalue approach , only linearised equilibrium is analyzed and non-linear behavior of the brake system is not taken into account .
	manualset3
94458	3	400570	13	NULL	NULL	0	NULL	non-linear behavior 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the complex eigenvalue approach , only linearised equilibrium is analyzed and non-linear behavior of the brake system is not taken into account .
	manualset3
94461	4	400570	13	NULL	NULL	0	NULL	brake system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In the complex eigenvalue approach , only linearised equilibrium is analyzed and non-linear behavior of the brake system is not taken into account .
	manualset3
94462	5	400570	13	NULL	NULL	0	NULL	account	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the complex eigenvalue approach , only linearised equilibrium is analyzed and non-linear behavior of the brake system is not taken into account .
	manualset3
94463	1	400571	13	NULL	NULL	0	NULL	Changes in the levels of oxidation-related substances	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	1 ) Changes in the levels of oxidation-related substances in blood , aqueous humor , and vitreous body from diabetic patients : all had decreased levels of reduced glutathione and superoxide scavenging activity , and increased levels of lipid peroxide and glycated protein .
	manualset3
94464	2	400571	13	NULL	NULL	0	NULL	blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	1 ) Changes in the levels of oxidation-related substances in blood , aqueous humor , and vitreous body from diabetic patients : all had decreased levels of reduced glutathione and superoxide scavenging activity , and increased levels of lipid peroxide and glycated protein .
	manualset3
94465	3	400571	13	NULL	NULL	0	NULL	aqueous humor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	1 ) Changes in the levels of oxidation-related substances in blood , aqueous humor , and vitreous body from diabetic patients : all had decreased levels of reduced glutathione and superoxide scavenging activity , and increased levels of lipid peroxide and glycated protein .
	manualset3
94466	4	400571	13	NULL	NULL	0	NULL	vitreous body 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	1 ) Changes in the levels of oxidation-related substances in blood , aqueous humor , and vitreous body from diabetic patients : all had decreased levels of reduced glutathione and superoxide scavenging activity , and increased levels of lipid peroxide and glycated protein .
	manualset3
94467	5	400571	13	NULL	NULL	0	NULL	diabetic patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	1 ) Changes in the levels of oxidation-related substances in blood , aqueous humor , and vitreous body from diabetic patients : all had decreased levels of reduced glutathione and superoxide scavenging activity , and increased levels of lipid peroxide and glycated protein .
	manualset3
94468	6	400571	13	NULL	NULL	0	NULL	levels of reduced glutathione	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	1 ) Changes in the levels of oxidation-related substances in blood , aqueous humor , and vitreous body from diabetic patients : all had decreased levels of reduced glutathione and superoxide scavenging activity , and increased levels of lipid peroxide and glycated protein .
	manualset3
94469	7	400571	13	NULL	NULL	0	NULL	superoxide scavenging activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	1 ) Changes in the levels of oxidation-related substances in blood , aqueous humor , and vitreous body from diabetic patients : all had decreased levels of reduced glutathione and superoxide scavenging activity , and increased levels of lipid peroxide and glycated protein .
	manualset3
94470	8	400571	13	NULL	NULL	0	NULL	 levels of lipid peroxide	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	1 ) Changes in the levels of oxidation-related substances in blood , aqueous humor , and vitreous body from diabetic patients : all had decreased levels of reduced glutathione and superoxide scavenging activity , and increased levels of lipid peroxide and glycated protein .
	manualset3
94471	9	400571	13	NULL	NULL	0	NULL	levels of glycated protein	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	1 ) Changes in the levels of oxidation-related substances in blood , aqueous humor , and vitreous body from diabetic patients : all had decreased levels of reduced glutathione and superoxide scavenging activity , and increased levels of lipid peroxide and glycated protein .
	manualset3
94472	1	400572	13	NULL	NULL	0	NULL	host	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the compromised host , the microbes most frequently associated with nosocomial infections in the ICU are bacteria that normally reside in or on body surfaces or in the environment .
	manualset3
94473	2	400572	13	NULL	NULL	0	NULL	microbes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the compromised host , the microbes most frequently associated with nosocomial infections in the ICU are bacteria that normally reside in or on body surfaces or in the environment .
	manualset3
94474	3	400572	13	NULL	NULL	0	NULL	nosocomial infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the compromised host , the microbes most frequently associated with nosocomial infections in the ICU are bacteria that normally reside in or on body surfaces or in the environment .
	manualset3
94475	4	400572	13	NULL	NULL	0	NULL	ICU 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In the compromised host , the microbes most frequently associated with nosocomial infections in the ICU are bacteria that normally reside in or on body surfaces or in the environment .
	manualset3
94476	5	400572	13	NULL	NULL	0	NULL	bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the compromised host , the microbes most frequently associated with nosocomial infections in the ICU are bacteria that normally reside in or on body surfaces or in the environment .
	manualset3
94477	6	400572	13	NULL	NULL	0	NULL	body surfaces	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the compromised host , the microbes most frequently associated with nosocomial infections in the ICU are bacteria that normally reside in or on body surfaces or in the environment .
	manualset3
94478	7	400572	13	NULL	NULL	0	NULL	environment	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In the compromised host , the microbes most frequently associated with nosocomial infections in the ICU are bacteria that normally reside in or on body surfaces or in the environment .
	manualset3
94479	1	400573	13	NULL	NULL	0	NULL	contact zone	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the contact zone , maternal ( megagametophtye ) and paternal ( embryo ) haplotypes were identified in 31 single seeds , demonstrating bidirectional pollen flow extending beyond the range of maternal haplotypes .
	manualset3
94480	2	400573	13	NULL	NULL	0	NULL	maternal ( megagametophtye ) haplotypes 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the contact zone , maternal ( megagametophtye ) and paternal ( embryo ) haplotypes were identified in 31 single seeds , demonstrating bidirectional pollen flow extending beyond the range of maternal haplotypes .
	manualset3
94481	3	400573	13	NULL	NULL	0	NULL	paternal ( embryo ) haplotypes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the contact zone , maternal ( megagametophtye ) and paternal ( embryo ) haplotypes were identified in 31 single seeds , demonstrating bidirectional pollen flow extending beyond the range of maternal haplotypes .
	manualset3
94482	4	400573	13	NULL	NULL	0	NULL	31	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the contact zone , maternal ( megagametophtye ) and paternal ( embryo ) haplotypes were identified in 31 single seeds , demonstrating bidirectional pollen flow extending beyond the range of maternal haplotypes .
	manualset3
94483	5	400573	13	NULL	NULL	0	NULL	single seeds	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the contact zone , maternal ( megagametophtye ) and paternal ( embryo ) haplotypes were identified in 31 single seeds , demonstrating bidirectional pollen flow extending beyond the range of maternal haplotypes .
	manualset3
94484	6	400573	13	NULL	NULL	0	NULL	bidirectional pollen flow	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the contact zone , maternal ( megagametophtye ) and paternal ( embryo ) haplotypes were identified in 31 single seeds , demonstrating bidirectional pollen flow extending beyond the range of maternal haplotypes .
	manualset3
94485	7	400573	13	NULL	NULL	0	NULL	range	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the contact zone , maternal ( megagametophtye ) and paternal ( embryo ) haplotypes were identified in 31 single seeds , demonstrating bidirectional pollen flow extending beyond the range of maternal haplotypes .
	manualset3
94486	8	400573	13	NULL	NULL	0	NULL	maternal haplotypes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the contact zone , maternal ( megagametophtye ) and paternal ( embryo ) haplotypes were identified in 31 single seeds , demonstrating bidirectional pollen flow extending beyond the range of maternal haplotypes .
	manualset3
94487	1	400574	13	NULL	NULL	0	NULL	conventional method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the conventional method , only the resultant contact force and the track drawn by the point of its application are considered so that the product of the instantaneous force and sliding increment is integrated over one motion cycle .
	manualset3
94488	2	400574	13	NULL	NULL	0	NULL	contact force	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the conventional method , only the resultant contact force and the track drawn by the point of its application are considered so that the product of the instantaneous force and sliding increment is integrated over one motion cycle .
	manualset3
94490	4	400574	13	NULL	NULL	0	NULL	point	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the conventional method , only the resultant contact force and the track drawn by the point of its application are considered so that the product of the instantaneous force and sliding increment is integrated over one motion cycle .
	manualset3
94491	5	400574	13	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the conventional method , only the resultant contact force and the track drawn by the point of its application are considered so that the product of the instantaneous force and sliding increment is integrated over one motion cycle .
	manualset3
94492	6	400574	13	NULL	NULL	0	NULL	product	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the conventional method , only the resultant contact force and the track drawn by the point of its application are considered so that the product of the instantaneous force and sliding increment is integrated over one motion cycle .
	manualset3
94493	7	400574	13	NULL	NULL	0	NULL	instantaneous force	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the conventional method , only the resultant contact force and the track drawn by the point of its application are considered so that the product of the instantaneous force and sliding increment is integrated over one motion cycle .
	manualset3
94494	8	400574	13	NULL	NULL	0	NULL	increment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the conventional method , only the resultant contact force and the track drawn by the point of its application are considered so that the product of the instantaneous force and sliding increment is integrated over one motion cycle .
	manualset3
94495	9	400574	13	NULL	NULL	0	NULL	one motion cycle 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the conventional method , only the resultant contact force and the track drawn by the point of its application are considered so that the product of the instantaneous force and sliding increment is integrated over one motion cycle .
	manualset3
94489	1	400575	13	NULL	NULL	NULL	NULL	corpus callosum 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the corpus callosum of the cat , the heavy subunit of neurofilaments ( NFH ) can be demonstrated with the monoclonal antibody NE14 , as early as P11 , not at P3 , and only in a few axons .
	manualset3
94496	2	400575	13	NULL	NULL	0	NULL	cat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the corpus callosum of the cat , the heavy subunit of neurofilaments ( NFH ) can be demonstrated with the monoclonal antibody NE14 , as early as P11 , not at P3 , and only in a few axons .
	manualset3
94497	3	400575	13	NULL	NULL	0	NULL	heavy subunit of neurofilaments ( NFH ) 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the corpus callosum of the cat , the heavy subunit of neurofilaments ( NFH ) can be demonstrated with the monoclonal antibody NE14 , as early as P11 , not at P3 , and only in a few axons .
	manualset3
94498	4	400575	13	NULL	NULL	0	NULL	monoclonal antibody NE14	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the corpus callosum of the cat , the heavy subunit of neurofilaments ( NFH ) can be demonstrated with the monoclonal antibody NE14 , as early as P11 , not at P3 , and only in a few axons .
	manualset3
94499	5	400575	13	NULL	NULL	0	NULL	P11	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the corpus callosum of the cat , the heavy subunit of neurofilaments ( NFH ) can be demonstrated with the monoclonal antibody NE14 , as early as P11 , not at P3 , and only in a few axons .
	manualset3
94500	6	400575	13	NULL	NULL	0	NULL	 P3 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the corpus callosum of the cat , the heavy subunit of neurofilaments ( NFH ) can be demonstrated with the monoclonal antibody NE14 , as early as P11 , not at P3 , and only in a few axons .
	manualset3
94501	7	400575	13	NULL	NULL	0	NULL	axons 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In the corpus callosum of the cat , the heavy subunit of neurofilaments ( NFH ) can be demonstrated with the monoclonal antibody NE14 , as early as P11 , not at P3 , and only in a few axons .
	manualset3
94541	1	400576	13	NULL	NULL	0	NULL	course	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the course of doing so , they have developed guidelines for gathering information , constructing goal scales , selecting expected outcome levels , and categorizing subsequent outcome data .
	manualset3
94542	2	400576	13	NULL	NULL	0	NULL	guidelines 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the course of doing so , they have developed guidelines for gathering information , constructing goal scales , selecting expected outcome levels , and categorizing subsequent outcome data .
	manualset3
94543	3	400576	13	NULL	NULL	0	NULL	gathering information	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the course of doing so , they have developed guidelines for gathering information , constructing goal scales , selecting expected outcome levels , and categorizing subsequent outcome data .
	manualset3
94544	4	400576	13	NULL	NULL	0	NULL	goal scales	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the course of doing so , they have developed guidelines for gathering information , constructing goal scales , selecting expected outcome levels , and categorizing subsequent outcome data .
	manualset3
94545	5	400576	13	NULL	NULL	0	NULL	outcome levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the course of doing so , they have developed guidelines for gathering information , constructing goal scales , selecting expected outcome levels , and categorizing subsequent outcome data .
	manualset3
94546	6	400576	13	NULL	NULL	0	NULL	subsequent outcome data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the course of doing so , they have developed guidelines for gathering information , constructing goal scales , selecting expected outcome levels , and categorizing subsequent outcome data .
	manualset3
94547	1	400577	13	NULL	NULL	0	NULL	course	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the course of optimizing CE separation conditions for FBP purified from cow 's milk we discovered a novel specific heparin-binding activity of FBP by affinity CE .
	manualset3
94548	2	400577	13	NULL	NULL	NULL	NULL	CE separation conditions	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the course of optimizing CE separation conditions for FBP purified from cow 's milk we discovered a novel specific heparin-binding activity of FBP by affinity CE .
	manualset3
94549	3	400577	13	NULL	NULL	NULL	NULL	FBP	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the course of optimizing CE separation conditions for FBP purified from cow 's milk we discovered a novel specific heparin-binding activity of FBP by affinity CE .
	manualset3
94550	4	400577	13	NULL	NULL	0	NULL	cow 's milk	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	In the course of optimizing CE separation conditions for FBP purified from cow 's milk we discovered a novel specific heparin-binding activity of FBP by affinity CE .
	manualset3
94551	5	400577	13	NULL	NULL	0	NULL	novel specific heparin-binding activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the course of optimizing CE separation conditions for FBP purified from cow 's milk we discovered a novel specific heparin-binding activity of FBP by affinity CE .
	manualset3
94552	6	400577	13	NULL	NULL	0	NULL	FBP 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the course of optimizing CE separation conditions for FBP purified from cow 's milk we discovered a novel specific heparin-binding activity of FBP by affinity CE .
	manualset3
94553	7	400577	13	NULL	NULL	0	NULL	 affinity CE	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the course of optimizing CE separation conditions for FBP purified from cow 's milk we discovered a novel specific heparin-binding activity of FBP by affinity CE .
	manualset3
94554	1	400578	13	NULL	NULL	0	NULL	course	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the course of our work on anti-platelet constituents from plants , five phenolic compounds , magnolol , honokiol , obovatol , methyl caffeate , and syringin , were isolated from the methanol extracts of the barks and fruits of Magnolia obovata .
	manualset3
94555	2	400578	13	NULL	NULL	0	NULL	work	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the course of our work on anti-platelet constituents from plants , five phenolic compounds , magnolol , honokiol , obovatol , methyl caffeate , and syringin , were isolated from the methanol extracts of the barks and fruits of Magnolia obovata .
	manualset3
94556	3	400578	13	NULL	NULL	0	NULL	anti-platelet constituents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the course of our work on anti-platelet constituents from plants , five phenolic compounds , magnolol , honokiol , obovatol , methyl caffeate , and syringin , were isolated from the methanol extracts of the barks and fruits of Magnolia obovata .
	manualset3
94558	4	400578	13	NULL	NULL	0	NULL	plants 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the course of our work on anti-platelet constituents from plants , five phenolic compounds , magnolol , honokiol , obovatol , methyl caffeate , and syringin , were isolated from the methanol extracts of the barks and fruits of Magnolia obovata .
	manualset3
94559	5	400578	13	NULL	NULL	0	NULL	five	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the course of our work on anti-platelet constituents from plants , five phenolic compounds , magnolol , honokiol , obovatol , methyl caffeate , and syringin , were isolated from the methanol extracts of the barks and fruits of Magnolia obovata .
	manualset3
94560	6	400578	13	NULL	NULL	0	NULL	phenolic compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the course of our work on anti-platelet constituents from plants , five phenolic compounds , magnolol , honokiol , obovatol , methyl caffeate , and syringin , were isolated from the methanol extracts of the barks and fruits of Magnolia obovata .
	manualset3
94561	7	400578	13	NULL	NULL	0	NULL	 magnolol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the course of our work on anti-platelet constituents from plants , five phenolic compounds , magnolol , honokiol , obovatol , methyl caffeate , and syringin , were isolated from the methanol extracts of the barks and fruits of Magnolia obovata .
	manualset3
94562	8	400578	13	NULL	NULL	0	NULL	honokiol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the course of our work on anti-platelet constituents from plants , five phenolic compounds , magnolol , honokiol , obovatol , methyl caffeate , and syringin , were isolated from the methanol extracts of the barks and fruits of Magnolia obovata .
	manualset3
94563	9	400578	13	NULL	NULL	0	NULL	obovatol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the course of our work on anti-platelet constituents from plants , five phenolic compounds , magnolol , honokiol , obovatol , methyl caffeate , and syringin , were isolated from the methanol extracts of the barks and fruits of Magnolia obovata .
	manualset3
94564	10	400578	13	NULL	NULL	0	NULL	methyl caffeate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the course of our work on anti-platelet constituents from plants , five phenolic compounds , magnolol , honokiol , obovatol , methyl caffeate , and syringin , were isolated from the methanol extracts of the barks and fruits of Magnolia obovata .
	manualset3
94565	11	400578	13	NULL	NULL	0	NULL	syringin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the course of our work on anti-platelet constituents from plants , five phenolic compounds , magnolol , honokiol , obovatol , methyl caffeate , and syringin , were isolated from the methanol extracts of the barks and fruits of Magnolia obovata .
	manualset3
94566	12	400578	13	NULL	NULL	0	NULL	methanol extracts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the course of our work on anti-platelet constituents from plants , five phenolic compounds , magnolol , honokiol , obovatol , methyl caffeate , and syringin , were isolated from the methanol extracts of the barks and fruits of Magnolia obovata .
	manualset3
94567	13	400578	13	NULL	NULL	0	NULL	barks	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the course of our work on anti-platelet constituents from plants , five phenolic compounds , magnolol , honokiol , obovatol , methyl caffeate , and syringin , were isolated from the methanol extracts of the barks and fruits of Magnolia obovata .
	manualset3
94568	14	400578	13	NULL	NULL	0	NULL	fruits	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the course of our work on anti-platelet constituents from plants , five phenolic compounds , magnolol , honokiol , obovatol , methyl caffeate , and syringin , were isolated from the methanol extracts of the barks and fruits of Magnolia obovata .
	manualset3
94569	15	400578	13	NULL	NULL	0	NULL	Magnolia obovata	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the course of our work on anti-platelet constituents from plants , five phenolic compounds , magnolol , honokiol , obovatol , methyl caffeate , and syringin , were isolated from the methanol extracts of the barks and fruits of Magnolia obovata .
	manualset3
94570	1	400579	13	NULL	NULL	0	NULL	crystal structure	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal structure , inter-molecular N-HO hydrogen bonds link the mol-ecules into centrosymmetric dimers ; these dimers are linked via inter-molecular O-HS hydrogen bonds , leading to infinite corrugated layers parallel to the bc plane through R ( 2 ) ( 2 ) ( 16 ) ring motifs .
	manualset3
94571	2	400579	13	NULL	NULL	0	NULL	 inter-molecular N-HO hydrogen bonds	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal structure , inter-molecular N-HO hydrogen bonds link the mol-ecules into centrosymmetric dimers ; these dimers are linked via inter-molecular O-HS hydrogen bonds , leading to infinite corrugated layers parallel to the bc plane through R ( 2 ) ( 2 ) ( 16 ) ring motifs .
	manualset3
94572	3	400579	13	NULL	NULL	NULL	NULL	mol-ecules	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the crystal structure , inter-molecular N-HO hydrogen bonds link the mol-ecules into centrosymmetric dimers ; these dimers are linked via inter-molecular O-HS hydrogen bonds , leading to infinite corrugated layers parallel to the bc plane through R ( 2 ) ( 2 ) ( 16 ) ring motifs .
	manualset3
94573	4	400579	13	NULL	NULL	0	NULL	centrosymmetric dimers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal structure , inter-molecular N-HO hydrogen bonds link the mol-ecules into centrosymmetric dimers ; these dimers are linked via inter-molecular O-HS hydrogen bonds , leading to infinite corrugated layers parallel to the bc plane through R ( 2 ) ( 2 ) ( 16 ) ring motifs .
	manualset3
94574	5	400579	13	NULL	NULL	0	NULL	dimers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal structure , inter-molecular N-HO hydrogen bonds link the mol-ecules into centrosymmetric dimers ; these dimers are linked via inter-molecular O-HS hydrogen bonds , leading to infinite corrugated layers parallel to the bc plane through R ( 2 ) ( 2 ) ( 16 ) ring motifs .
	manualset3
94575	6	400579	13	NULL	NULL	0	NULL	inter-molecular O-HS hydrogen bonds	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal structure , inter-molecular N-HO hydrogen bonds link the mol-ecules into centrosymmetric dimers ; these dimers are linked via inter-molecular O-HS hydrogen bonds , leading to infinite corrugated layers parallel to the bc plane through R ( 2 ) ( 2 ) ( 16 ) ring motifs .
	manualset3
94576	7	400579	13	NULL	NULL	0	NULL	 infinite corrugated layers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal structure , inter-molecular N-HO hydrogen bonds link the mol-ecules into centrosymmetric dimers ; these dimers are linked via inter-molecular O-HS hydrogen bonds , leading to infinite corrugated layers parallel to the bc plane through R ( 2 ) ( 2 ) ( 16 ) ring motifs .
	manualset3
94577	8	400579	13	NULL	NULL	0	NULL	 bc plane	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal structure , inter-molecular N-HO hydrogen bonds link the mol-ecules into centrosymmetric dimers ; these dimers are linked via inter-molecular O-HS hydrogen bonds , leading to infinite corrugated layers parallel to the bc plane through R ( 2 ) ( 2 ) ( 16 ) ring motifs .
	manualset3
94578	9	400579	13	NULL	NULL	0	NULL	R ( 2 ) ( 2 ) ( 16 ) ring motifs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal structure , inter-molecular N-HO hydrogen bonds link the mol-ecules into centrosymmetric dimers ; these dimers are linked via inter-molecular O-HS hydrogen bonds , leading to infinite corrugated layers parallel to the bc plane through R ( 2 ) ( 2 ) ( 16 ) ring motifs .
	manualset3
94579	1	400580	13	NULL	NULL	0	NULL	Approaches	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Approaches to low-income groups ' sexuality : a comparative study of women in three low-income contexts in Peru ) .
	manualset3
94580	2	400580	13	NULL	NULL	0	NULL	low-income groups '	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Approaches to low-income groups ' sexuality : a comparative study of women in three low-income contexts in Peru ) .
	manualset3
94581	3	400580	13	NULL	NULL	0	NULL	sexuality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Approaches to low-income groups ' sexuality : a comparative study of women in three low-income contexts in Peru ) .
	manualset3
94582	4	400580	13	NULL	NULL	0	NULL	a comparative study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Approaches to low-income groups ' sexuality : a comparative study of women in three low-income contexts in Peru ) .
	manualset3
94583	5	400580	13	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Approaches to low-income groups ' sexuality : a comparative study of women in three low-income contexts in Peru ) .
	manualset3
94584	6	400580	13	NULL	NULL	0	NULL	 three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Approaches to low-income groups ' sexuality : a comparative study of women in three low-income contexts in Peru ) .
	manualset3
94585	7	400580	13	NULL	NULL	0	NULL	low-income contexts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Approaches to low-income groups ' sexuality : a comparative study of women in three low-income contexts in Peru ) .
	manualset3
94586	8	400580	13	NULL	NULL	0	NULL	Peru 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Approaches to low-income groups ' sexuality : a comparative study of women in three low-income contexts in Peru ) .
	manualset3
94587	1	400581	13	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	1 ) The amount , hardness , and histological findings concerning the remaining hematoma differed markedly according to which hematolytic agents were used .
	manualset3
94588	2	400581	13	NULL	NULL	0	NULL	hardness 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	1 ) The amount , hardness , and histological findings concerning the remaining hematoma differed markedly according to which hematolytic agents were used .
	manualset3
94589	3	400581	13	NULL	NULL	0	NULL	 histological findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	1 ) The amount , hardness , and histological findings concerning the remaining hematoma differed markedly according to which hematolytic agents were used .
	manualset3
94590	4	400581	13	NULL	NULL	0	NULL	hematoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	1 ) The amount , hardness , and histological findings concerning the remaining hematoma differed markedly according to which hematolytic agents were used .
	manualset3
94591	5	400581	13	NULL	NULL	0	NULL	hematolytic agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	1 ) The amount , hardness , and histological findings concerning the remaining hematoma differed markedly according to which hematolytic agents were used .
	manualset3
94592	1	400582	13	NULL	NULL	0	NULL	crystal structure	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal structure , inter-molecular N-HO hydrogen bonds link the mol-ecules into infinite chains along the c axis .
	manualset3
94593	2	400582	13	NULL	NULL	0	NULL	 inter-molecular N-HO hydrogen bonds	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal structure , inter-molecular N-HO hydrogen bonds link the mol-ecules into infinite chains along the c axis .
	manualset3
94594	3	400582	13	NULL	NULL	0	NULL	 mol-ecules 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal structure , inter-molecular N-HO hydrogen bonds link the mol-ecules into infinite chains along the c axis .
	manualset3
94595	4	400582	13	NULL	NULL	0	NULL	 infinite chains 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal structure , inter-molecular N-HO hydrogen bonds link the mol-ecules into infinite chains along the c axis .
	manualset3
94596	5	400582	13	NULL	NULL	0	NULL	c axis	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal structure , inter-molecular N-HO hydrogen bonds link the mol-ecules into infinite chains along the c axis .
	manualset3
94597	1	400583	13	NULL	NULL	0	NULL	crystal 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal , mol-ecules are linked by N-HO hydrogen bonds and weak C-HO inter-actions into tapes along the b axis .
	manualset3
94598	2	400583	13	NULL	NULL	0	NULL	mol-ecules	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal , mol-ecules are linked by N-HO hydrogen bonds and weak C-HO inter-actions into tapes along the b axis .
	manualset3
94599	3	400583	13	NULL	NULL	0	NULL	N-HO hydrogen bonds	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal , mol-ecules are linked by N-HO hydrogen bonds and weak C-HO inter-actions into tapes along the b axis .
	manualset3
94600	4	400583	13	NULL	NULL	0	NULL	weak C-HO inter-actions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal , mol-ecules are linked by N-HO hydrogen bonds and weak C-HO inter-actions into tapes along the b axis .
	manualset3
94601	5	400583	13	NULL	NULL	0	NULL	tapes along the b axis	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal , mol-ecules are linked by N-HO hydrogen bonds and weak C-HO inter-actions into tapes along the b axis .
	manualset3
94602	1	400584	13	NULL	NULL	0	NULL	crystal 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal , each solvent mol-ecule is linked to the metal complex by weak inter-molecular C-HO hydrogen bonds .
	manualset3
94603	2	400584	13	NULL	NULL	0	NULL	solvent mol-ecule	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal , each solvent mol-ecule is linked to the metal complex by weak inter-molecular C-HO hydrogen bonds .
	manualset3
94604	3	400584	13	NULL	NULL	0	NULL	 metal complex	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal , each solvent mol-ecule is linked to the metal complex by weak inter-molecular C-HO hydrogen bonds .
	manualset3
94605	4	400584	13	NULL	NULL	0	NULL	weak inter-molecular C-HO hydrogen bonds	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal , each solvent mol-ecule is linked to the metal complex by weak inter-molecular C-HO hydrogen bonds .
	manualset3
94606	1	400585	13	NULL	NULL	0	NULL	cuneate nucleus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cuneate nucleus , single injections in the hand produced dense label in the pars rotunda , and sparse label in the rostral and caudal poles .
	manualset3
94607	2	400585	13	NULL	NULL	0	NULL	single injections 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cuneate nucleus , single injections in the hand produced dense label in the pars rotunda , and sparse label in the rostral and caudal poles .
	manualset3
94608	3	400585	13	NULL	NULL	0	NULL	hand	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cuneate nucleus , single injections in the hand produced dense label in the pars rotunda , and sparse label in the rostral and caudal poles .
	manualset3
94609	4	400585	13	NULL	NULL	0	NULL	dense label	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cuneate nucleus , single injections in the hand produced dense label in the pars rotunda , and sparse label in the rostral and caudal poles .
	manualset3
94610	5	400585	13	NULL	NULL	0	NULL	pars rotunda	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cuneate nucleus , single injections in the hand produced dense label in the pars rotunda , and sparse label in the rostral and caudal poles .
	manualset3
94611	6	400585	13	NULL	NULL	0	NULL	sparse label	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cuneate nucleus , single injections in the hand produced dense label in the pars rotunda , and sparse label in the rostral and caudal poles .
	manualset3
94612	7	400585	13	NULL	NULL	0	NULL	rostral poles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cuneate nucleus , single injections in the hand produced dense label in the pars rotunda , and sparse label in the rostral and caudal poles .
	manualset3
94613	8	400585	13	NULL	NULL	0	NULL	caudal poles 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cuneate nucleus , single injections in the hand produced dense label in the pars rotunda , and sparse label in the rostral and caudal poles .
	manualset3
94614	1	400586	13	NULL	NULL	0	NULL	current literature review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current literature review , both generic and breast cancer specific QOL instruments , examining computerized and paper-and-pencil versions , are explained as well as the advantages , acceptability , and problems of these assessments .
	manualset3
94615	2	400586	13	NULL	NULL	0	NULL	breast cancer specific QOL instruments	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current literature review , both generic and breast cancer specific QOL instruments , examining computerized and paper-and-pencil versions , are explained as well as the advantages , acceptability , and problems of these assessments .
	manualset3
94616	3	400586	13	NULL	NULL	0	NULL	paper-and-pencil versions	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current literature review , both generic and breast cancer specific QOL instruments , examining computerized and paper-and-pencil versions , are explained as well as the advantages , acceptability , and problems of these assessments .
	manualset3
94617	4	400586	13	NULL	NULL	NULL	NULL	advantages	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the current literature review , both generic and breast cancer specific QOL instruments , examining computerized and paper-and-pencil versions , are explained as well as the advantages , acceptability , and problems of these assessments .
	manualset3
94618	5	400586	13	NULL	NULL	0	NULL	acceptability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current literature review , both generic and breast cancer specific QOL instruments , examining computerized and paper-and-pencil versions , are explained as well as the advantages , acceptability , and problems of these assessments .
	manualset3
94619	6	400586	13	NULL	NULL	0	NULL	problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current literature review , both generic and breast cancer specific QOL instruments , examining computerized and paper-and-pencil versions , are explained as well as the advantages , acceptability , and problems of these assessments .
	manualset3
94620	7	400586	13	NULL	NULL	0	NULL	assessments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current literature review , both generic and breast cancer specific QOL instruments , examining computerized and paper-and-pencil versions , are explained as well as the advantages , acceptability , and problems of these assessments .
	manualset3
98580	8	400586	13	NULL	NULL	0	NULL	computerized versions	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current literature review , both generic and breast cancer specific QOL instruments , examining computerized and paper-and-pencil versions , are explained as well as the advantages , acceptability , and problems of these assessments .
	manualset3
94621	1	400587	13	NULL	NULL	0	NULL	 current study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current study , it was shown that 244/PR8 also protects against disease caused by a heterologous influenza B virus ( B/Lee/40 ) .
	manualset3
94622	2	400587	13	NULL	NULL	0	NULL	244/PR8 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current study , it was shown that 244/PR8 also protects against disease caused by a heterologous influenza B virus ( B/Lee/40 ) .
	manualset3
94623	3	400587	13	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current study , it was shown that 244/PR8 also protects against disease caused by a heterologous influenza B virus ( B/Lee/40 ) .
	manualset3
94624	4	400587	13	NULL	NULL	0	NULL	heterologous influenza B virus ( B/Lee/40 )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current study , it was shown that 244/PR8 also protects against disease caused by a heterologous influenza B virus ( B/Lee/40 ) .
	manualset3
94625	1	400588	13	NULL	NULL	0	NULL	current study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current study , we aim to characterize the nature of changes in EphB1 receptor expression following increases or decreases in dopamine activity .
	manualset3
94626	2	400588	13	NULL	NULL	0	NULL	nature of changes 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current study , we aim to characterize the nature of changes in EphB1 receptor expression following increases or decreases in dopamine activity .
	manualset3
94627	3	400588	13	NULL	NULL	0	NULL	EphB1 receptor expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current study , we aim to characterize the nature of changes in EphB1 receptor expression following increases or decreases in dopamine activity .
	manualset3
94628	4	400588	13	NULL	NULL	0	NULL	dopamine activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current study , we aim to characterize the nature of changes in EphB1 receptor expression following increases or decreases in dopamine activity .
	manualset3
94629	1	400589	13	NULL	NULL	0	NULL	current study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current study , we examine depression among men and women aged 18-75 in 23 European countries .
	manualset3
94630	2	400589	13	NULL	NULL	0	NULL	depression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current study , we examine depression among men and women aged 18-75 in 23 European countries .
	manualset3
94631	3	400589	13	NULL	NULL	0	NULL	men aged 18-75	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current study , we examine depression among men and women aged 18-75 in 23 European countries .
	manualset3
94632	4	400589	13	NULL	NULL	0	NULL	women aged 18-75	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current study , we examine depression among men and women aged 18-75 in 23 European countries .
	manualset3
94633	5	400589	13	NULL	NULL	0	NULL	23 European countries	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current study , we examine depression among men and women aged 18-75 in 23 European countries .
	manualset3
94634	1	400590	13	NULL	NULL	0	NULL	 current study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current study , we investigated the regulation of expression of the A3 AR gene , focusing on sequences conserved in the mouse and human promoters .
	manualset3
94635	2	400590	13	NULL	NULL	0	NULL	regulation of expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current study , we investigated the regulation of expression of the A3 AR gene , focusing on sequences conserved in the mouse and human promoters .
	manualset3
94636	3	400590	13	NULL	NULL	0	NULL	A3 AR gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current study , we investigated the regulation of expression of the A3 AR gene , focusing on sequences conserved in the mouse and human promoters .
	manualset3
94638	5	400590	13	NULL	NULL	0	NULL	sequences 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current study , we investigated the regulation of expression of the A3 AR gene , focusing on sequences conserved in the mouse and human promoters .
	manualset3
94639	6	400590	13	NULL	NULL	0	NULL	mouse promoters  	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current study , we investigated the regulation of expression of the A3 AR gene , focusing on sequences conserved in the mouse and human promoters .
	manualset3
94640	7	400590	13	NULL	NULL	0	NULL	human promoters 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current study , we investigated the regulation of expression of the A3 AR gene , focusing on sequences conserved in the mouse and human promoters .
	manualset3
94641	1	400591	13	NULL	NULL	0	NULL	cytoplasm 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cytoplasm , fractionation , dilation , and vesiculation of rough endoplasmic reticulum ( RER ) , and elevated amounts of smooth endoplasmic reticulum ( SER ) tubules were noted .
	manualset3
94642	2	400591	13	NULL	NULL	NULL	NULL	 fractionation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the cytoplasm , fractionation , dilation , and vesiculation of rough endoplasmic reticulum ( RER ) , and elevated amounts of smooth endoplasmic reticulum ( SER ) tubules were noted .
	manualset3
94643	3	400591	13	NULL	NULL	0	NULL	 dilation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cytoplasm , fractionation , dilation , and vesiculation of rough endoplasmic reticulum ( RER ) , and elevated amounts of smooth endoplasmic reticulum ( SER ) tubules were noted .
	manualset3
94644	4	400591	13	NULL	NULL	0	NULL	vesiculation of rough endoplasmic reticulum ( RER )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cytoplasm , fractionation , dilation , and vesiculation of rough endoplasmic reticulum ( RER ) , and elevated amounts of smooth endoplasmic reticulum ( SER ) tubules were noted .
	manualset3
94645	5	400591	13	NULL	NULL	0	NULL	amounts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cytoplasm , fractionation , dilation , and vesiculation of rough endoplasmic reticulum ( RER ) , and elevated amounts of smooth endoplasmic reticulum ( SER ) tubules were noted .
	manualset3
94646	6	400591	13	NULL	NULL	0	NULL	smooth endoplasmic reticulum ( SER ) tubules 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cytoplasm , fractionation , dilation , and vesiculation of rough endoplasmic reticulum ( RER ) , and elevated amounts of smooth endoplasmic reticulum ( SER ) tubules were noted .
	manualset3
94647	1	400592	13	NULL	NULL	NULL	NULL	cell suspension	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the diluted cell suspension , single cardiomyocytes and capillary fragments containing 6-15 endothelial cells could be identified morphologically .
	manualset3
94648	2	400592	13	NULL	NULL	0	NULL	cardiomyocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the diluted cell suspension , single cardiomyocytes and capillary fragments containing 6-15 endothelial cells could be identified morphologically .
	manualset3
94649	3	400592	13	NULL	NULL	0	NULL	capillary fragments	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the diluted cell suspension , single cardiomyocytes and capillary fragments containing 6-15 endothelial cells could be identified morphologically .
	manualset3
94650	4	400592	13	NULL	NULL	0	NULL	6-15 endothelial cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the diluted cell suspension , single cardiomyocytes and capillary fragments containing 6-15 endothelial cells could be identified morphologically .
	manualset3
94651	1	400593	13	NULL	NULL	0	NULL	drug-sensitivity test	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the drug-sensitivity test , the combination therapy also exerted strong activity .
	manualset3
94652	2	400593	13	NULL	NULL	0	NULL	combination therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the drug-sensitivity test , the combination therapy also exerted strong activity .
	manualset3
94653	3	400593	13	NULL	NULL	0	NULL	strong activity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the drug-sensitivity test , the combination therapy also exerted strong activity .
	manualset3
94654	1	400594	13	NULL	NULL	0	NULL	early 1960s	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In the early 1960s , health care professionals were attracted to the new insights of cytogenetics , including the chromosomal explanation of Down syndrome and of other congenital defects and abnormalities of sexual development .
	manualset3
94655	2	400594	13	NULL	NULL	0	NULL	 health care professionals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the early 1960s , health care professionals were attracted to the new insights of cytogenetics , including the chromosomal explanation of Down syndrome and of other congenital defects and abnormalities of sexual development .
	manualset3
94656	3	400594	13	NULL	NULL	0	NULL	 new insights of cytogenetics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In the early 1960s , health care professionals were attracted to the new insights of cytogenetics , including the chromosomal explanation of Down syndrome and of other congenital defects and abnormalities of sexual development .
	manualset3
94657	4	400594	13	NULL	NULL	0	NULL	chromosomal explanation of Down syndrome	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In the early 1960s , health care professionals were attracted to the new insights of cytogenetics , including the chromosomal explanation of Down syndrome and of other congenital defects and abnormalities of sexual development .
	manualset3
94658	5	400594	13	NULL	NULL	0	NULL	congenital defects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the early 1960s , health care professionals were attracted to the new insights of cytogenetics , including the chromosomal explanation of Down syndrome and of other congenital defects and abnormalities of sexual development .
	manualset3
94659	6	400594	13	NULL	NULL	0	NULL	abnormalities of sexual development	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the early 1960s , health care professionals were attracted to the new insights of cytogenetics , including the chromosomal explanation of Down syndrome and of other congenital defects and abnormalities of sexual development .
	manualset3
94660	1	400595	13	NULL	NULL	0	NULL	 early stages	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the early stages of apoptosis changes occur at the cell surface , which until now have remained difficult to recognize .
	manualset3
94661	2	400595	13	NULL	NULL	0	NULL	apoptosis changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the early stages of apoptosis changes occur at the cell surface , which until now have remained difficult to recognize .
	manualset3
94662	3	400595	13	NULL	NULL	0	NULL	cell surface	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In the early stages of apoptosis changes occur at the cell surface , which until now have remained difficult to recognize .
	manualset3
94663	1	400596	13	NULL	NULL	0	NULL	 eight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the eight patients with inducible PSVT before and after disopyramide , tachycardia cycle length increased from 348 + / - 33 to 404 + / - 29 msec ( mean + / - SEM ) ( p less than 0.001 ) .
	manualset3
94664	2	400596	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the eight patients with inducible PSVT before and after disopyramide , tachycardia cycle length increased from 348 + / - 33 to 404 + / - 29 msec ( mean + / - SEM ) ( p less than 0.001 ) .
	manualset3
94665	3	400596	13	NULL	NULL	0	NULL	inducible PSVT	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the eight patients with inducible PSVT before and after disopyramide , tachycardia cycle length increased from 348 + / - 33 to 404 + / - 29 msec ( mean + / - SEM ) ( p less than 0.001 ) .
	manualset3
94666	4	400596	13	NULL	NULL	0	NULL	disopyramide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the eight patients with inducible PSVT before and after disopyramide , tachycardia cycle length increased from 348 + / - 33 to 404 + / - 29 msec ( mean + / - SEM ) ( p less than 0.001 ) .
	manualset3
94667	5	400596	13	NULL	NULL	0	NULL	 tachycardia cycle length	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the eight patients with inducible PSVT before and after disopyramide , tachycardia cycle length increased from 348 + / - 33 to 404 + / - 29 msec ( mean + / - SEM ) ( p less than 0.001 ) .
	manualset3
94668	6	400596	13	NULL	NULL	0	NULL	348 + / - 33 to 404 + / - 29 msec ( mean + / - SEM ) ( p less than 0.001 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the eight patients with inducible PSVT before and after disopyramide , tachycardia cycle length increased from 348 + / - 33 to 404 + / - 29 msec ( mean + / - SEM ) ( p less than 0.001 ) .
	manualset3
94669	1	400597	13	NULL	NULL	0	NULL	micronutrient deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the elderly , micronutrient deficiency is a common presenting clinical picture ; because the symptoms of malabsorption are covert , the diagnosis often is delayed , and nutritional deficiencies are more common and more severe than in the young .
	manualset3
94670	2	400597	13	NULL	NULL	0	NULL	clinical picture	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the elderly , micronutrient deficiency is a common presenting clinical picture ; because the symptoms of malabsorption are covert , the diagnosis often is delayed , and nutritional deficiencies are more common and more severe than in the young .
	manualset3
94671	3	400597	13	NULL	NULL	0	NULL	symptoms of malabsorption	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the elderly , micronutrient deficiency is a common presenting clinical picture ; because the symptoms of malabsorption are covert , the diagnosis often is delayed , and nutritional deficiencies are more common and more severe than in the young .
	manualset3
94672	4	400597	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the elderly , micronutrient deficiency is a common presenting clinical picture ; because the symptoms of malabsorption are covert , the diagnosis often is delayed , and nutritional deficiencies are more common and more severe than in the young .
	manualset3
94673	5	400597	13	NULL	NULL	0	NULL	nutritional deficiencies 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the elderly , micronutrient deficiency is a common presenting clinical picture ; because the symptoms of malabsorption are covert , the diagnosis often is delayed , and nutritional deficiencies are more common and more severe than in the young .
	manualset3
94674	6	400597	13	NULL	NULL	0	NULL	 young	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the elderly , micronutrient deficiency is a common presenting clinical picture ; because the symptoms of malabsorption are covert , the diagnosis often is delayed , and nutritional deficiencies are more common and more severe than in the young .
	manualset3
98581	7	400597	13	NULL	NULL	0	NULL	elderly 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the elderly , micronutrient deficiency is a common presenting clinical picture ; because the symptoms of malabsorption are covert , the diagnosis often is delayed , and nutritional deficiencies are more common and more severe than in the young .
	manualset3
94675	1	400598	13	NULL	NULL	0	NULL	Leukotrienes	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	1 Leukotrienes constitute a class of potent bioactive mediators known to play a pivotal role in inflammation .
	manualset3
94676	2	400598	13	NULL	NULL	0	NULL	class of potent bioactive mediators 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	1 Leukotrienes constitute a class of potent bioactive mediators known to play a pivotal role in inflammation .
	manualset3
94677	3	400598	13	NULL	NULL	0	NULL	pivotal role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	1 Leukotrienes constitute a class of potent bioactive mediators known to play a pivotal role in inflammation .
	manualset3
94678	4	400598	13	NULL	NULL	0	NULL	inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	1 Leukotrienes constitute a class of potent bioactive mediators known to play a pivotal role in inflammation .
	manualset3
94679	1	400599	13	NULL	NULL	0	NULL	estimation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the estimation of REE using the Harris-Benedict formula , a correction factor ( 1.1 ) should be considered to accurately assess energy needs .
	manualset3
94680	2	400599	13	NULL	NULL	0	NULL	REE	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the estimation of REE using the Harris-Benedict formula , a correction factor ( 1.1 ) should be considered to accurately assess energy needs .
	manualset3
94681	3	400599	13	NULL	NULL	0	NULL	Harris-Benedict formula	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In the estimation of REE using the Harris-Benedict formula , a correction factor ( 1.1 ) should be considered to accurately assess energy needs .
	manualset3
94682	4	400599	13	NULL	NULL	0	NULL	correction factor ( 1.1 )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the estimation of REE using the Harris-Benedict formula , a correction factor ( 1.1 ) should be considered to accurately assess energy needs .
	manualset3
94683	5	400599	13	NULL	NULL	0	NULL	energy needs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the estimation of REE using the Harris-Benedict formula , a correction factor ( 1.1 ) should be considered to accurately assess energy needs .
	manualset3
94684	1	400600	13	NULL	NULL	0	NULL	field of social sciences	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In the field of social sciences , there has been a renewed interest in studying prejudice and discrimination as stressors and assessing their impact on various health outcomes .
	manualset3
94685	2	400600	13	NULL	NULL	0	NULL	interest 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the field of social sciences , there has been a renewed interest in studying prejudice and discrimination as stressors and assessing their impact on various health outcomes .
	manualset3
94686	3	400600	13	NULL	NULL	0	NULL	prejudice	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the field of social sciences , there has been a renewed interest in studying prejudice and discrimination as stressors and assessing their impact on various health outcomes .
	manualset3
94687	4	400600	13	NULL	NULL	NULL	NULL	discrimination	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the field of social sciences , there has been a renewed interest in studying prejudice and discrimination as stressors and assessing their impact on various health outcomes .
	manualset3
94688	5	400600	13	NULL	NULL	NULL	NULL	stressors	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the field of social sciences , there has been a renewed interest in studying prejudice and discrimination as stressors and assessing their impact on various health outcomes .
	manualset3
94689	6	400600	13	NULL	NULL	0	NULL	impact	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the field of social sciences , there has been a renewed interest in studying prejudice and discrimination as stressors and assessing their impact on various health outcomes .
	manualset3
94690	7	400600	13	NULL	NULL	0	NULL	various health outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the field of social sciences , there has been a renewed interest in studying prejudice and discrimination as stressors and assessing their impact on various health outcomes .
	manualset3
94691	1	400601	13	NULL	NULL	0	NULL	2 weeks 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the final 2 weeks changes in fiber intakes were : Gp A , mean increase 7.2 + / - 1.0 g per day ( P less than 0.001 ) ; Gp B , mean increase 9.1 + / - 1.6 g per day ( P less than 0.001 ) ; Gp C mean decrease 3.50 + / - 1.6 g per day ( P less than 0.005 ) .
	manualset3
94692	2	400601	13	NULL	NULL	0	NULL	changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the final 2 weeks changes in fiber intakes were : Gp A , mean increase 7.2 + / - 1.0 g per day ( P less than 0.001 ) ; Gp B , mean increase 9.1 + / - 1.6 g per day ( P less than 0.001 ) ; Gp C mean decrease 3.50 + / - 1.6 g per day ( P less than 0.005 ) .
	manualset3
94693	3	400601	13	NULL	NULL	0	NULL	fiber intakes 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	In the final 2 weeks changes in fiber intakes were : Gp A , mean increase 7.2 + / - 1.0 g per day ( P less than 0.001 ) ; Gp B , mean increase 9.1 + / - 1.6 g per day ( P less than 0.001 ) ; Gp C mean decrease 3.50 + / - 1.6 g per day ( P less than 0.005 ) .
	manualset3
94694	4	400601	13	NULL	NULL	0	NULL	 Gp A	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the final 2 weeks changes in fiber intakes were : Gp A , mean increase 7.2 + / - 1.0 g per day ( P less than 0.001 ) ; Gp B , mean increase 9.1 + / - 1.6 g per day ( P less than 0.001 ) ; Gp C mean decrease 3.50 + / - 1.6 g per day ( P less than 0.005 ) .
	manualset3
94695	5	400601	13	NULL	NULL	0	NULL	 mean increase 7.2 + / - 1.0 g per day ( P less than 0.001 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the final 2 weeks changes in fiber intakes were : Gp A , mean increase 7.2 + / - 1.0 g per day ( P less than 0.001 ) ; Gp B , mean increase 9.1 + / - 1.6 g per day ( P less than 0.001 ) ; Gp C mean decrease 3.50 + / - 1.6 g per day ( P less than 0.005 ) .
	manualset3
94696	6	400601	13	NULL	NULL	0	NULL	Gp B	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the final 2 weeks changes in fiber intakes were : Gp A , mean increase 7.2 + / - 1.0 g per day ( P less than 0.001 ) ; Gp B , mean increase 9.1 + / - 1.6 g per day ( P less than 0.001 ) ; Gp C mean decrease 3.50 + / - 1.6 g per day ( P less than 0.005 ) .
	manualset3
94697	7	400601	13	NULL	NULL	0	NULL	mean increase 9.1 + / - 1.6 g per day ( P less than 0.001 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the final 2 weeks changes in fiber intakes were : Gp A , mean increase 7.2 + / - 1.0 g per day ( P less than 0.001 ) ; Gp B , mean increase 9.1 + / - 1.6 g per day ( P less than 0.001 ) ; Gp C mean decrease 3.50 + / - 1.6 g per day ( P less than 0.005 ) .
	manualset3
94698	8	400601	13	NULL	NULL	0	NULL	Gp C	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the final 2 weeks changes in fiber intakes were : Gp A , mean increase 7.2 + / - 1.0 g per day ( P less than 0.001 ) ; Gp B , mean increase 9.1 + / - 1.6 g per day ( P less than 0.001 ) ; Gp C mean decrease 3.50 + / - 1.6 g per day ( P less than 0.005 ) .
	manualset3
94699	9	400601	13	NULL	NULL	0	NULL	mean decrease 3.50 + / - 1.6 g per day ( P less than 0.005 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the final 2 weeks changes in fiber intakes were : Gp A , mean increase 7.2 + / - 1.0 g per day ( P less than 0.001 ) ; Gp B , mean increase 9.1 + / - 1.6 g per day ( P less than 0.001 ) ; Gp C mean decrease 3.50 + / - 1.6 g per day ( P less than 0.005 ) .
	manualset3
94700	1	400602	13	NULL	NULL	0	NULL	bone powders	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the fine particulate bone powders , Sry was detected all the time and its expression was statistically greater than in the larger bone grafts at each time point .
	manualset3
94701	2	400602	13	NULL	NULL	0	NULL	Sry 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the fine particulate bone powders , Sry was detected all the time and its expression was statistically greater than in the larger bone grafts at each time point .
	manualset3
94702	3	400602	13	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In the fine particulate bone powders , Sry was detected all the time and its expression was statistically greater than in the larger bone grafts at each time point .
	manualset3
94703	4	400602	13	NULL	NULL	0	NULL	 expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the fine particulate bone powders , Sry was detected all the time and its expression was statistically greater than in the larger bone grafts at each time point .
	manualset3
94704	5	400602	13	NULL	NULL	0	NULL	larger bone grafts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the fine particulate bone powders , Sry was detected all the time and its expression was statistically greater than in the larger bone grafts at each time point .
	manualset3
94705	6	400602	13	NULL	NULL	NULL	NULL	each time point	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the fine particulate bone powders , Sry was detected all the time and its expression was statistically greater than in the larger bone grafts at each time point .
	manualset3
94706	1	400603	13	NULL	NULL	0	NULL	first case	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In the first case the problem of the missing upper lateral incisors was solved by adhesive bridges , after the fixed appliance orthodontic treatment , where the diasthema medianum was closed , and the upper canines were distalized .
	manualset3
94707	2	400603	13	NULL	NULL	0	NULL	problem of the missing upper lateral incisors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the first case the problem of the missing upper lateral incisors was solved by adhesive bridges , after the fixed appliance orthodontic treatment , where the diasthema medianum was closed , and the upper canines were distalized .
	manualset3
94708	3	400603	13	NULL	NULL	0	NULL	adhesive bridges	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the first case the problem of the missing upper lateral incisors was solved by adhesive bridges , after the fixed appliance orthodontic treatment , where the diasthema medianum was closed , and the upper canines were distalized .
	manualset3
94709	4	400603	13	NULL	NULL	0	NULL	appliance orthodontic treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the first case the problem of the missing upper lateral incisors was solved by adhesive bridges , after the fixed appliance orthodontic treatment , where the diasthema medianum was closed , and the upper canines were distalized .
	manualset3
94710	5	400603	13	NULL	NULL	0	NULL	diasthema medianum 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the first case the problem of the missing upper lateral incisors was solved by adhesive bridges , after the fixed appliance orthodontic treatment , where the diasthema medianum was closed , and the upper canines were distalized .
	manualset3
94711	6	400603	13	NULL	NULL	0	NULL	upper canines	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the first case the problem of the missing upper lateral incisors was solved by adhesive bridges , after the fixed appliance orthodontic treatment , where the diasthema medianum was closed , and the upper canines were distalized .
	manualset3
94712	1	400604	13	NULL	NULL	0	NULL	first experiment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the first experiment , bradycardia ( -54 beat/min ) was observed in unrestrained 2-day Sprague-Dawley rat pups 2.5 h after treatment with the adrenergic neuron blocking agent bretylium tosylate , indicating that sympathetic neural control of basal heart rate is functional in newborn rats .
	manualset3
94713	2	400604	13	NULL	NULL	0	NULL	 bradycardia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the first experiment , bradycardia ( -54 beat/min ) was observed in unrestrained 2-day Sprague-Dawley rat pups 2.5 h after treatment with the adrenergic neuron blocking agent bretylium tosylate , indicating that sympathetic neural control of basal heart rate is functional in newborn rats .
	manualset3
94714	3	400604	13	NULL	NULL	0	NULL	-54 beat/min 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the first experiment , bradycardia ( -54 beat/min ) was observed in unrestrained 2-day Sprague-Dawley rat pups 2.5 h after treatment with the adrenergic neuron blocking agent bretylium tosylate , indicating that sympathetic neural control of basal heart rate is functional in newborn rats .
	manualset3
94715	4	400604	13	NULL	NULL	0	NULL	unrestrained 2-day Sprague-Dawley rat pups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the first experiment , bradycardia ( -54 beat/min ) was observed in unrestrained 2-day Sprague-Dawley rat pups 2.5 h after treatment with the adrenergic neuron blocking agent bretylium tosylate , indicating that sympathetic neural control of basal heart rate is functional in newborn rats .
	manualset3
94716	5	400604	13	NULL	NULL	0	NULL	2.5 h 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the first experiment , bradycardia ( -54 beat/min ) was observed in unrestrained 2-day Sprague-Dawley rat pups 2.5 h after treatment with the adrenergic neuron blocking agent bretylium tosylate , indicating that sympathetic neural control of basal heart rate is functional in newborn rats .
	manualset3
94717	6	400604	13	NULL	NULL	0	NULL	 treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the first experiment , bradycardia ( -54 beat/min ) was observed in unrestrained 2-day Sprague-Dawley rat pups 2.5 h after treatment with the adrenergic neuron blocking agent bretylium tosylate , indicating that sympathetic neural control of basal heart rate is functional in newborn rats .
	manualset3
94718	7	400604	13	NULL	NULL	0	NULL	 adrenergic neuron blocking agent	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the first experiment , bradycardia ( -54 beat/min ) was observed in unrestrained 2-day Sprague-Dawley rat pups 2.5 h after treatment with the adrenergic neuron blocking agent bretylium tosylate , indicating that sympathetic neural control of basal heart rate is functional in newborn rats .
	manualset3
94719	8	400604	13	NULL	NULL	0	NULL	bretylium tosylate	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the first experiment , bradycardia ( -54 beat/min ) was observed in unrestrained 2-day Sprague-Dawley rat pups 2.5 h after treatment with the adrenergic neuron blocking agent bretylium tosylate , indicating that sympathetic neural control of basal heart rate is functional in newborn rats .
	manualset3
94720	9	400604	13	NULL	NULL	0	NULL	sympathetic neural control of basal heart rate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the first experiment , bradycardia ( -54 beat/min ) was observed in unrestrained 2-day Sprague-Dawley rat pups 2.5 h after treatment with the adrenergic neuron blocking agent bretylium tosylate , indicating that sympathetic neural control of basal heart rate is functional in newborn rats .
	manualset3
94721	10	400604	13	NULL	NULL	0	NULL	newborn rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the first experiment , bradycardia ( -54 beat/min ) was observed in unrestrained 2-day Sprague-Dawley rat pups 2.5 h after treatment with the adrenergic neuron blocking agent bretylium tosylate , indicating that sympathetic neural control of basal heart rate is functional in newborn rats .
	manualset3
94722	1	400605	13	NULL	NULL	0	NULL	 first study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the first study , the effect of RMP-7 on enhancing the BBB permeation of three compounds of different physical characteristics was directly compared ( ( 14C ) carboplatin , small , hydrophilic ; ( 14C ) dextran , large , hydrophilic ; ( 14C ) BCNU , small , lipophilic ) .
	manualset3
94723	2	400605	13	NULL	NULL	0	NULL	effect of RMP-7	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the first study , the effect of RMP-7 on enhancing the BBB permeation of three compounds of different physical characteristics was directly compared ( ( 14C ) carboplatin , small , hydrophilic ; ( 14C ) dextran , large , hydrophilic ; ( 14C ) BCNU , small , lipophilic ) .
	manualset3
94724	3	400605	13	NULL	NULL	0	NULL	BBB permeation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the first study , the effect of RMP-7 on enhancing the BBB permeation of three compounds of different physical characteristics was directly compared ( ( 14C ) carboplatin , small , hydrophilic ; ( 14C ) dextran , large , hydrophilic ; ( 14C ) BCNU , small , lipophilic ) .
	manualset3
94725	4	400605	13	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the first study , the effect of RMP-7 on enhancing the BBB permeation of three compounds of different physical characteristics was directly compared ( ( 14C ) carboplatin , small , hydrophilic ; ( 14C ) dextran , large , hydrophilic ; ( 14C ) BCNU , small , lipophilic ) .
	manualset3
94726	5	400605	13	NULL	NULL	0	NULL	compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the first study , the effect of RMP-7 on enhancing the BBB permeation of three compounds of different physical characteristics was directly compared ( ( 14C ) carboplatin , small , hydrophilic ; ( 14C ) dextran , large , hydrophilic ; ( 14C ) BCNU , small , lipophilic ) .
	manualset3
94727	6	400605	13	NULL	NULL	NULL	NULL	physical characteristics	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the first study , the effect of RMP-7 on enhancing the BBB permeation of three compounds of different physical characteristics was directly compared ( ( 14C ) carboplatin , small , hydrophilic ; ( 14C ) dextran , large , hydrophilic ; ( 14C ) BCNU , small , lipophilic ) .
	manualset3
94728	7	400605	13	NULL	NULL	0	NULL	( 14C ) carboplatin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the first study , the effect of RMP-7 on enhancing the BBB permeation of three compounds of different physical characteristics was directly compared ( ( 14C ) carboplatin , small , hydrophilic ; ( 14C ) dextran , large , hydrophilic ; ( 14C ) BCNU , small , lipophilic ) .
	manualset3
94729	8	400605	13	NULL	NULL	0	NULL	( 14C ) dextran 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the first study , the effect of RMP-7 on enhancing the BBB permeation of three compounds of different physical characteristics was directly compared ( ( 14C ) carboplatin , small , hydrophilic ; ( 14C ) dextran , large , hydrophilic ; ( 14C ) BCNU , small , lipophilic ) .
	manualset3
94730	9	400605	13	NULL	NULL	0	NULL	( 14C ) BCNU	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the first study , the effect of RMP-7 on enhancing the BBB permeation of three compounds of different physical characteristics was directly compared ( ( 14C ) carboplatin , small , hydrophilic ; ( 14C ) dextran , large , hydrophilic ; ( 14C ) BCNU , small , lipophilic ) .
	manualset3
94731	1	400606	13	NULL	NULL	0	NULL	activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	1 The activity produced by intra-arterial bradykinin and prostaglandin E1 was investigated in multifibre strands dissected from the saphenous nerves of anaesthetized rats .
	manualset3
94732	2	400606	13	NULL	NULL	0	NULL	 intra-arterial bradykinin	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	1 The activity produced by intra-arterial bradykinin and prostaglandin E1 was investigated in multifibre strands dissected from the saphenous nerves of anaesthetized rats .
	manualset3
94733	3	400606	13	NULL	NULL	0	NULL	prostaglandin E1	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	1 The activity produced by intra-arterial bradykinin and prostaglandin E1 was investigated in multifibre strands dissected from the saphenous nerves of anaesthetized rats .
	manualset3
94734	4	400606	13	NULL	NULL	0	NULL	multifibre strands	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	1 The activity produced by intra-arterial bradykinin and prostaglandin E1 was investigated in multifibre strands dissected from the saphenous nerves of anaesthetized rats .
	manualset3
94735	5	400606	13	NULL	NULL	0	NULL	saphenous nerves	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	1 The activity produced by intra-arterial bradykinin and prostaglandin E1 was investigated in multifibre strands dissected from the saphenous nerves of anaesthetized rats .
	manualset3
94736	6	400606	13	NULL	NULL	0	NULL	rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	1 The activity produced by intra-arterial bradykinin and prostaglandin E1 was investigated in multifibre strands dissected from the saphenous nerves of anaesthetized rats .
	manualset3
94737	1	400607	13	NULL	NULL	0	NULL	first type , the mutation ( tynP )	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the first type , the mutation ( tynP ) was closely linked to the structural gene for tyramine oxidase tynA ) .
	manualset3
94738	2	400607	13	NULL	NULL	0	NULL	structural gene for tyramine oxidase tynA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In the first type , the mutation ( tynP ) was closely linked to the structural gene for tyramine oxidase tynA ) .
	manualset3
94739	1	400608	13	NULL	NULL	0	NULL	four 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the four examined tissues , the myostatin gene was highly expressed in muscle and intestine and weakly expressed in brain and liver .
	manualset3
94740	2	400608	13	NULL	NULL	0	NULL	tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In the four examined tissues , the myostatin gene was highly expressed in muscle and intestine and weakly expressed in brain and liver .
	manualset3
94741	3	400608	13	NULL	NULL	0	NULL	 myostatin gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In the four examined tissues , the myostatin gene was highly expressed in muscle and intestine and weakly expressed in brain and liver .
	manualset3
94742	4	400608	13	NULL	NULL	0	NULL	muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the four examined tissues , the myostatin gene was highly expressed in muscle and intestine and weakly expressed in brain and liver .
	manualset3
94743	5	400608	13	NULL	NULL	0	NULL	intestine 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the four examined tissues , the myostatin gene was highly expressed in muscle and intestine and weakly expressed in brain and liver .
	manualset3
94744	6	400608	13	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the four examined tissues , the myostatin gene was highly expressed in muscle and intestine and weakly expressed in brain and liver .
	manualset3
94745	7	400608	13	NULL	NULL	0	NULL	 liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the four examined tissues , the myostatin gene was highly expressed in muscle and intestine and weakly expressed in brain and liver .
	manualset3
94746	1	400609	13	NULL	NULL	0	NULL	future	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In the future , the safety of blood components may be increased by testing donated blood by nucleic acid amplification techniques and by photochemical decontamination of cellular blood components .
	manualset3
94747	2	400609	13	NULL	NULL	NULL	NULL	safety	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the future , the safety of blood components may be increased by testing donated blood by nucleic acid amplification techniques and by photochemical decontamination of cellular blood components .
	manualset3
94748	3	400609	13	NULL	NULL	0	NULL	blood components 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the future , the safety of blood components may be increased by testing donated blood by nucleic acid amplification techniques and by photochemical decontamination of cellular blood components .
	manualset3
94749	4	400609	13	NULL	NULL	0	NULL	testing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the future , the safety of blood components may be increased by testing donated blood by nucleic acid amplification techniques and by photochemical decontamination of cellular blood components .
	manualset3
94750	5	400609	13	NULL	NULL	0	NULL	blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In the future , the safety of blood components may be increased by testing donated blood by nucleic acid amplification techniques and by photochemical decontamination of cellular blood components .
	manualset3
94751	6	400609	13	NULL	NULL	0	NULL	nucleic acid amplification techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the future , the safety of blood components may be increased by testing donated blood by nucleic acid amplification techniques and by photochemical decontamination of cellular blood components .
	manualset3
94752	7	400609	13	NULL	NULL	0	NULL	photochemical decontamination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the future , the safety of blood components may be increased by testing donated blood by nucleic acid amplification techniques and by photochemical decontamination of cellular blood components .
	manualset3
94753	8	400609	13	NULL	NULL	0	NULL	cellular blood components	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the future , the safety of blood components may be increased by testing donated blood by nucleic acid amplification techniques and by photochemical decontamination of cellular blood components .
	manualset3
94754	1	400610	13	NULL	NULL	0	NULL	future 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In the future , this technique could be optimized to examine specific genes instrumental in fetal organ system function , which could be a useful addition to prenatal care .
	manualset3
94755	2	400610	13	NULL	NULL	0	NULL	technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the future , this technique could be optimized to examine specific genes instrumental in fetal organ system function , which could be a useful addition to prenatal care .
	manualset3
94756	3	400610	13	NULL	NULL	0	NULL	genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the future , this technique could be optimized to examine specific genes instrumental in fetal organ system function , which could be a useful addition to prenatal care .
	manualset3
94757	4	400610	13	NULL	NULL	0	NULL	fetal organ system function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the future , this technique could be optimized to examine specific genes instrumental in fetal organ system function , which could be a useful addition to prenatal care .
	manualset3
94758	5	400610	13	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the future , this technique could be optimized to examine specific genes instrumental in fetal organ system function , which could be a useful addition to prenatal care .
	manualset3
94759	6	400610	13	NULL	NULL	0	NULL	prenatal care	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the future , this technique could be optimized to examine specific genes instrumental in fetal organ system function , which could be a useful addition to prenatal care .
	manualset3
94760	1	400611	13	NULL	NULL	NULL	NULL	general game theoretic approach 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the general game theoretic approach , the behavior of conspecifics is included in the determination of the distinguished organism 's strategy .
	manualset3
94762	3	400611	13	NULL	NULL	0	NULL	behavior of conspecifics	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the general game theoretic approach , the behavior of conspecifics is included in the determination of the distinguished organism 's strategy .
	manualset3
94763	4	400611	13	NULL	NULL	0	NULL	determination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the general game theoretic approach , the behavior of conspecifics is included in the determination of the distinguished organism 's strategy .
	manualset3
94764	5	400611	13	NULL	NULL	0	NULL	organism 's strategy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the general game theoretic approach , the behavior of conspecifics is included in the determination of the distinguished organism 's strategy .
	manualset3
94765	1	400612	13	NULL	NULL	0	NULL	group of patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the group of patients subjected to coronarography where three arteries or the trunk of the left coronary artery was affected the score in 81.8 % of the patients was smaller than -10 .
	manualset3
94766	2	400612	13	NULL	NULL	0	NULL	coronarography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the group of patients subjected to coronarography where three arteries or the trunk of the left coronary artery was affected the score in 81.8 % of the patients was smaller than -10 .
	manualset3
94767	3	400612	13	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the group of patients subjected to coronarography where three arteries or the trunk of the left coronary artery was affected the score in 81.8 % of the patients was smaller than -10 .
	manualset3
94768	4	400612	13	NULL	NULL	0	NULL	arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the group of patients subjected to coronarography where three arteries or the trunk of the left coronary artery was affected the score in 81.8 % of the patients was smaller than -10 .
	manualset3
94769	5	400612	13	NULL	NULL	0	NULL	trunk of the left coronary artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the group of patients subjected to coronarography where three arteries or the trunk of the left coronary artery was affected the score in 81.8 % of the patients was smaller than -10 .
	manualset3
94770	6	400612	13	NULL	NULL	NULL	NULL	score	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the group of patients subjected to coronarography where three arteries or the trunk of the left coronary artery was affected the score in 81.8 % of the patients was smaller than -10 .
	manualset3
94771	8	400612	13	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the group of patients subjected to coronarography where three arteries or the trunk of the left coronary artery was affected the score in 81.8 % of the patients was smaller than -10 .
	manualset3
94772	9	400612	13	NULL	NULL	NULL	NULL	smaller than -10	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the group of patients subjected to coronarography where three arteries or the trunk of the left coronary artery was affected the score in 81.8 % of the patients was smaller than -10 .
	manualset3
94773	7	400612	13	NULL	NULL	0	NULL	81.8 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the group of patients subjected to coronarography where three arteries or the trunk of the left coronary artery was affected the score in 81.8 % of the patients was smaller than -10 .
	manualset3
94774	1	400613	13	NULL	NULL	0	NULL	effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	1 The effects of alkaline diuresis on the elimination of a single oral dose of 750 mg diflunisal were studied in six healthy male volunteers .
	manualset3
94775	2	400613	13	NULL	NULL	0	NULL	alkaline diuresis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	1 The effects of alkaline diuresis on the elimination of a single oral dose of 750 mg diflunisal were studied in six healthy male volunteers .
	manualset3
94776	3	400613	13	NULL	NULL	0	NULL	elimination 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	1 The effects of alkaline diuresis on the elimination of a single oral dose of 750 mg diflunisal were studied in six healthy male volunteers .
	manualset3
94777	4	400613	13	NULL	NULL	0	NULL	single oral dose	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	1 The effects of alkaline diuresis on the elimination of a single oral dose of 750 mg diflunisal were studied in six healthy male volunteers .
	manualset3
94778	5	400613	13	NULL	NULL	0	NULL	750 mg diflunisal	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	1 The effects of alkaline diuresis on the elimination of a single oral dose of 750 mg diflunisal were studied in six healthy male volunteers .
	manualset3
94779	6	400613	13	NULL	NULL	0	NULL	 six	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	1 The effects of alkaline diuresis on the elimination of a single oral dose of 750 mg diflunisal were studied in six healthy male volunteers .
	manualset3
94780	7	400613	13	NULL	NULL	0	NULL	healthy male volunteers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	1 The effects of alkaline diuresis on the elimination of a single oral dose of 750 mg diflunisal were studied in six healthy male volunteers .
	manualset3
94781	1	400614	13	NULL	NULL	NULL	NULL	 group with trauma	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the group with trauma the frequency of this phenomenon was increased compared to the group without trauma .
	manualset3
94783	2	400614	13	NULL	NULL	NULL	NULL	frequency	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the group with trauma the frequency of this phenomenon was increased compared to the group without trauma .
	manualset3
94784	3	400614	13	NULL	NULL	NULL	NULL	 phenomenon 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the group with trauma the frequency of this phenomenon was increased compared to the group without trauma .
	manualset3
94785	4	400614	13	NULL	NULL	NULL	NULL	group without trauma	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the group with trauma the frequency of this phenomenon was increased compared to the group without trauma .
	manualset3
94787	1	400615	13	NULL	NULL	0	NULL	guinea pig spinal cord	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the guinea pig spinal cord , LTC4 levels reached a peak concentration of 2.2 + / - 0.4 pmol/g cord 10 minutes after compression , while that of TXB2 reached 146.8 + / - 6.2 pmol/g cord .
	manualset3
94788	2	400615	13	NULL	NULL	0	NULL	LTC4 levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the guinea pig spinal cord , LTC4 levels reached a peak concentration of 2.2 + / - 0.4 pmol/g cord 10 minutes after compression , while that of TXB2 reached 146.8 + / - 6.2 pmol/g cord .
	manualset3
94789	3	400615	13	NULL	NULL	0	NULL	peak concentration of 2.2 + / - 0.4 pmol/g cord 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the guinea pig spinal cord , LTC4 levels reached a peak concentration of 2.2 + / - 0.4 pmol/g cord 10 minutes after compression , while that of TXB2 reached 146.8 + / - 6.2 pmol/g cord .
	manualset3
94790	4	400615	13	NULL	NULL	0	NULL	10 minutes	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In the guinea pig spinal cord , LTC4 levels reached a peak concentration of 2.2 + / - 0.4 pmol/g cord 10 minutes after compression , while that of TXB2 reached 146.8 + / - 6.2 pmol/g cord .
	manualset3
94791	5	400615	13	NULL	NULL	0	NULL	compression	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the guinea pig spinal cord , LTC4 levels reached a peak concentration of 2.2 + / - 0.4 pmol/g cord 10 minutes after compression , while that of TXB2 reached 146.8 + / - 6.2 pmol/g cord .
	manualset3
94792	6	400615	13	NULL	NULL	0	NULL	TXB2 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the guinea pig spinal cord , LTC4 levels reached a peak concentration of 2.2 + / - 0.4 pmol/g cord 10 minutes after compression , while that of TXB2 reached 146.8 + / - 6.2 pmol/g cord .
	manualset3
94793	7	400615	13	NULL	NULL	0	NULL	146.8 + / - 6.2 pmol/g cord 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the guinea pig spinal cord , LTC4 levels reached a peak concentration of 2.2 + / - 0.4 pmol/g cord 10 minutes after compression , while that of TXB2 reached 146.8 + / - 6.2 pmol/g cord .
	manualset3
94794	1	400616	13	NULL	NULL	0	NULL	human isolated bronchus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the human isolated bronchus , the offset of the bronchodilator effects of glycopyrrolate ( 3 nM ) , tiotropium ( 1 nM ) and ipratropium ( 10 nM ) was t1/2 = 3.7 + / - 0.2 ; ) 6 and 3.0 + / - 0.2 h , respectively .
	manualset3
94795	2	400616	13	NULL	NULL	0	NULL	bronchodilator effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the human isolated bronchus , the offset of the bronchodilator effects of glycopyrrolate ( 3 nM ) , tiotropium ( 1 nM ) and ipratropium ( 10 nM ) was t1/2 = 3.7 + / - 0.2 ; ) 6 and 3.0 + / - 0.2 h , respectively .
	manualset3
94796	3	400616	13	NULL	NULL	0	NULL	glycopyrrolate ( 3 nM )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the human isolated bronchus , the offset of the bronchodilator effects of glycopyrrolate ( 3 nM ) , tiotropium ( 1 nM ) and ipratropium ( 10 nM ) was t1/2 = 3.7 + / - 0.2 ; ) 6 and 3.0 + / - 0.2 h , respectively .
	manualset3
94797	4	400616	13	NULL	NULL	0	NULL	tiotropium ( 1 nM )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the human isolated bronchus , the offset of the bronchodilator effects of glycopyrrolate ( 3 nM ) , tiotropium ( 1 nM ) and ipratropium ( 10 nM ) was t1/2 = 3.7 + / - 0.2 ; ) 6 and 3.0 + / - 0.2 h , respectively .
	manualset3
94798	5	400616	13	NULL	NULL	0	NULL	ipratropium ( 10 nM )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the human isolated bronchus , the offset of the bronchodilator effects of glycopyrrolate ( 3 nM ) , tiotropium ( 1 nM ) and ipratropium ( 10 nM ) was t1/2 = 3.7 + / - 0.2 ; ) 6 and 3.0 + / - 0.2 h , respectively .
	manualset3
94799	6	400616	13	NULL	NULL	0	NULL	t1/2 = 3.7 + / - 0.2 h 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the human isolated bronchus , the offset of the bronchodilator effects of glycopyrrolate ( 3 nM ) , tiotropium ( 1 nM ) and ipratropium ( 10 nM ) was t1/2 = 3.7 + / - 0.2 ; ) 6 and 3.0 + / - 0.2 h , respectively .
	manualset3
94800	7	400616	13	NULL	NULL	0	NULL	t1/2> 6h	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the human isolated bronchus , the offset of the bronchodilator effects of glycopyrrolate ( 3 nM ) , tiotropium ( 1 nM ) and ipratropium ( 10 nM ) was t1/2 = 3.7 + / - 0.2 ; ) 6 and 3.0 + / - 0.2 h , respectively .
	manualset3
94801	8	400616	13	NULL	NULL	0	NULL	t1/2 = 3.0 + / - 0.2 h	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the human isolated bronchus , the offset of the bronchodilator effects of glycopyrrolate ( 3 nM ) , tiotropium ( 1 nM ) and ipratropium ( 10 nM ) was t1/2 = 3.7 + / - 0.2 ; ) 6 and 3.0 + / - 0.2 h , respectively .
	manualset3
94802	1	400617	13	NULL	NULL	0	NULL	humoral in vitro test 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the humoral in vitro test all the peptides act as stimulators .
	manualset3
94803	2	400617	13	NULL	NULL	0	NULL	peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	In the humoral in vitro test all the peptides act as stimulators .
	manualset3
94804	3	400617	13	NULL	NULL	0	NULL	stimulators	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the humoral in vitro test all the peptides act as stimulators .
	manualset3
94805	1	400618	13	NULL	NULL	NULL	NULL	hypothalamus	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the hypothalamus , there appeared a moderate immunoreaction for IgG , but no expression of iNOS .
	manualset3
94806	2	400618	13	NULL	NULL	0	NULL	 moderate immunoreaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the hypothalamus , there appeared a moderate immunoreaction for IgG , but no expression of iNOS .
	manualset3
94807	3	400618	13	NULL	NULL	0	NULL	IgG	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the hypothalamus , there appeared a moderate immunoreaction for IgG , but no expression of iNOS .
	manualset3
94808	4	400618	13	NULL	NULL	0	NULL	expression of iNOS	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the hypothalamus , there appeared a moderate immunoreaction for IgG , but no expression of iNOS .
	manualset3
94809	1	400619	13	NULL	NULL	0	NULL	ileum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the ileum , the m-to-s but not the s-to-m flux of 5-FU was reduced by ( 1 ) serosal ouabain ( 0.1 mM ) ; ( 2 ) reduction of the bathing solution Na concentration ; and ( 3 ) addition of uracil , thymine , thymidine , uridine , 2-deoxyuridine , or uridine-5 ' - monophosphate .
	manualset3
94810	2	400619	13	NULL	NULL	0	NULL	m-to-s flux of 5-FU	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the ileum , the m-to-s but not the s-to-m flux of 5-FU was reduced by ( 1 ) serosal ouabain ( 0.1 mM ) ; ( 2 ) reduction of the bathing solution Na concentration ; and ( 3 ) addition of uracil , thymine , thymidine , uridine , 2-deoxyuridine , or uridine-5 ' - monophosphate .
	manualset3
94811	3	400619	13	NULL	NULL	0	NULL	s-to-m flux of 5-FU	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the ileum , the m-to-s but not the s-to-m flux of 5-FU was reduced by ( 1 ) serosal ouabain ( 0.1 mM ) ; ( 2 ) reduction of the bathing solution Na concentration ; and ( 3 ) addition of uracil , thymine , thymidine , uridine , 2-deoxyuridine , or uridine-5 ' - monophosphate .
	manualset3
94812	4	400619	13	NULL	NULL	0	NULL	serosal ouabain ( 0.1 mM )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the ileum , the m-to-s but not the s-to-m flux of 5-FU was reduced by ( 1 ) serosal ouabain ( 0.1 mM ) ; ( 2 ) reduction of the bathing solution Na concentration ; and ( 3 ) addition of uracil , thymine , thymidine , uridine , 2-deoxyuridine , or uridine-5 ' - monophosphate .
	manualset3
94813	5	400619	13	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the ileum , the m-to-s but not the s-to-m flux of 5-FU was reduced by ( 1 ) serosal ouabain ( 0.1 mM ) ; ( 2 ) reduction of the bathing solution Na concentration ; and ( 3 ) addition of uracil , thymine , thymidine , uridine , 2-deoxyuridine , or uridine-5 ' - monophosphate .
	manualset3
94814	6	400619	13	NULL	NULL	NULL	NULL	bathing solution Na concentration	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the ileum , the m-to-s but not the s-to-m flux of 5-FU was reduced by ( 1 ) serosal ouabain ( 0.1 mM ) ; ( 2 ) reduction of the bathing solution Na concentration ; and ( 3 ) addition of uracil , thymine , thymidine , uridine , 2-deoxyuridine , or uridine-5 ' - monophosphate .
	manualset3
94815	7	400619	13	NULL	NULL	0	NULL	uracil	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the ileum , the m-to-s but not the s-to-m flux of 5-FU was reduced by ( 1 ) serosal ouabain ( 0.1 mM ) ; ( 2 ) reduction of the bathing solution Na concentration ; and ( 3 ) addition of uracil , thymine , thymidine , uridine , 2-deoxyuridine , or uridine-5 ' - monophosphate .
	manualset3
94816	8	400619	13	NULL	NULL	0	NULL	thymine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the ileum , the m-to-s but not the s-to-m flux of 5-FU was reduced by ( 1 ) serosal ouabain ( 0.1 mM ) ; ( 2 ) reduction of the bathing solution Na concentration ; and ( 3 ) addition of uracil , thymine , thymidine , uridine , 2-deoxyuridine , or uridine-5 ' - monophosphate .
	manualset3
94817	9	400619	13	NULL	NULL	0	NULL	thymidine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the ileum , the m-to-s but not the s-to-m flux of 5-FU was reduced by ( 1 ) serosal ouabain ( 0.1 mM ) ; ( 2 ) reduction of the bathing solution Na concentration ; and ( 3 ) addition of uracil , thymine , thymidine , uridine , 2-deoxyuridine , or uridine-5 ' - monophosphate .
	manualset3
94818	10	400619	13	NULL	NULL	0	NULL	uridine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the ileum , the m-to-s but not the s-to-m flux of 5-FU was reduced by ( 1 ) serosal ouabain ( 0.1 mM ) ; ( 2 ) reduction of the bathing solution Na concentration ; and ( 3 ) addition of uracil , thymine , thymidine , uridine , 2-deoxyuridine , or uridine-5 ' - monophosphate .
	manualset3
94819	11	400619	13	NULL	NULL	0	NULL	 2-deoxyuridine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the ileum , the m-to-s but not the s-to-m flux of 5-FU was reduced by ( 1 ) serosal ouabain ( 0.1 mM ) ; ( 2 ) reduction of the bathing solution Na concentration ; and ( 3 ) addition of uracil , thymine , thymidine , uridine , 2-deoxyuridine , or uridine-5 ' - monophosphate .
	manualset3
94820	12	400619	13	NULL	NULL	0	NULL	uridine-5 ' - monophosphate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the ileum , the m-to-s but not the s-to-m flux of 5-FU was reduced by ( 1 ) serosal ouabain ( 0.1 mM ) ; ( 2 ) reduction of the bathing solution Na concentration ; and ( 3 ) addition of uracil , thymine , thymidine , uridine , 2-deoxyuridine , or uridine-5 ' - monophosphate .
	manualset3
94821	1	400620	13	NULL	NULL	0	NULL	immunoprecipitation analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the immunoprecipitation analysis , the poly ( A ) - binding protein ( PABP ) and the RNA-binding protein HuR were pulled down by 3 ' - UTR cRNA , and the absence of the ARE site reduced the binding of these proteins .
	manualset3
94822	2	400620	13	NULL	NULL	0	NULL	poly ( A ) - binding protein ( PABP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the immunoprecipitation analysis , the poly ( A ) - binding protein ( PABP ) and the RNA-binding protein HuR were pulled down by 3 ' - UTR cRNA , and the absence of the ARE site reduced the binding of these proteins .
	manualset3
94823	3	400620	13	NULL	NULL	0	NULL	RNA-binding protein HuR 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the immunoprecipitation analysis , the poly ( A ) - binding protein ( PABP ) and the RNA-binding protein HuR were pulled down by 3 ' - UTR cRNA , and the absence of the ARE site reduced the binding of these proteins .
	manualset3
94824	4	400620	13	NULL	NULL	0	NULL	 3 ' - UTR cRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the immunoprecipitation analysis , the poly ( A ) - binding protein ( PABP ) and the RNA-binding protein HuR were pulled down by 3 ' - UTR cRNA , and the absence of the ARE site reduced the binding of these proteins .
	manualset3
94825	5	400620	13	NULL	NULL	0	NULL	ARE site 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the immunoprecipitation analysis , the poly ( A ) - binding protein ( PABP ) and the RNA-binding protein HuR were pulled down by 3 ' - UTR cRNA , and the absence of the ARE site reduced the binding of these proteins .
	manualset3
94826	6	400620	13	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the immunoprecipitation analysis , the poly ( A ) - binding protein ( PABP ) and the RNA-binding protein HuR were pulled down by 3 ' - UTR cRNA , and the absence of the ARE site reduced the binding of these proteins .
	manualset3
94827	7	400620	13	NULL	NULL	0	NULL	proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the immunoprecipitation analysis , the poly ( A ) - binding protein ( PABP ) and the RNA-binding protein HuR were pulled down by 3 ' - UTR cRNA , and the absence of the ARE site reduced the binding of these proteins .
	manualset3
94828	1	400621	13	NULL	NULL	0	NULL	 anti-inflammatory activity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	1 To investigate anti-inflammatory activity of organic germanium , we measured the effect of germanium-concentrated yeast on arachidonic acid release , prostaglandin E ( 2 ) ( PGE ( 2 ) ) production , histamine release , and intracellular H ( 2 ) O ( 2 ) or hydroperoxide generation in RBL 2H3 cells , and carrageenan-induced paw oedema in rats .
	manualset3
94829	2	400621	13	NULL	NULL	0	NULL	organic germanium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	1 To investigate anti-inflammatory activity of organic germanium , we measured the effect of germanium-concentrated yeast on arachidonic acid release , prostaglandin E ( 2 ) ( PGE ( 2 ) ) production , histamine release , and intracellular H ( 2 ) O ( 2 ) or hydroperoxide generation in RBL 2H3 cells , and carrageenan-induced paw oedema in rats .
	manualset3
94830	3	400621	13	NULL	NULL	0	NULL	 effect of germanium-concentrated yeast	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	1 To investigate anti-inflammatory activity of organic germanium , we measured the effect of germanium-concentrated yeast on arachidonic acid release , prostaglandin E ( 2 ) ( PGE ( 2 ) ) production , histamine release , and intracellular H ( 2 ) O ( 2 ) or hydroperoxide generation in RBL 2H3 cells , and carrageenan-induced paw oedema in rats .
	manualset3
94831	4	400621	13	NULL	NULL	0	NULL	arachidonic acid release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	1 To investigate anti-inflammatory activity of organic germanium , we measured the effect of germanium-concentrated yeast on arachidonic acid release , prostaglandin E ( 2 ) ( PGE ( 2 ) ) production , histamine release , and intracellular H ( 2 ) O ( 2 ) or hydroperoxide generation in RBL 2H3 cells , and carrageenan-induced paw oedema in rats .
	manualset3
94832	5	400621	13	NULL	NULL	0	NULL	prostaglandin E ( 2 ) ( PGE ( 2 ) ) production 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	1 To investigate anti-inflammatory activity of organic germanium , we measured the effect of germanium-concentrated yeast on arachidonic acid release , prostaglandin E ( 2 ) ( PGE ( 2 ) ) production , histamine release , and intracellular H ( 2 ) O ( 2 ) or hydroperoxide generation in RBL 2H3 cells , and carrageenan-induced paw oedema in rats .
	manualset3
94833	6	400621	13	NULL	NULL	0	NULL	histamine release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	1 To investigate anti-inflammatory activity of organic germanium , we measured the effect of germanium-concentrated yeast on arachidonic acid release , prostaglandin E ( 2 ) ( PGE ( 2 ) ) production , histamine release , and intracellular H ( 2 ) O ( 2 ) or hydroperoxide generation in RBL 2H3 cells , and carrageenan-induced paw oedema in rats .
	manualset3
94834	7	400621	13	NULL	NULL	0	NULL	 intracellular H ( 2 ) O ( 2 ) or hydroperoxide generation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	1 To investigate anti-inflammatory activity of organic germanium , we measured the effect of germanium-concentrated yeast on arachidonic acid release , prostaglandin E ( 2 ) ( PGE ( 2 ) ) production , histamine release , and intracellular H ( 2 ) O ( 2 ) or hydroperoxide generation in RBL 2H3 cells , and carrageenan-induced paw oedema in rats .
	manualset3
94835	8	400621	13	NULL	NULL	0	NULL	RBL 2H3 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	1 To investigate anti-inflammatory activity of organic germanium , we measured the effect of germanium-concentrated yeast on arachidonic acid release , prostaglandin E ( 2 ) ( PGE ( 2 ) ) production , histamine release , and intracellular H ( 2 ) O ( 2 ) or hydroperoxide generation in RBL 2H3 cells , and carrageenan-induced paw oedema in rats .
	manualset3
94836	9	400621	13	NULL	NULL	0	NULL	carrageenan-induced paw oedema 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	1 To investigate anti-inflammatory activity of organic germanium , we measured the effect of germanium-concentrated yeast on arachidonic acid release , prostaglandin E ( 2 ) ( PGE ( 2 ) ) production , histamine release , and intracellular H ( 2 ) O ( 2 ) or hydroperoxide generation in RBL 2H3 cells , and carrageenan-induced paw oedema in rats .
	manualset3
94837	10	400621	13	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	1 To investigate anti-inflammatory activity of organic germanium , we measured the effect of germanium-concentrated yeast on arachidonic acid release , prostaglandin E ( 2 ) ( PGE ( 2 ) ) production , histamine release , and intracellular H ( 2 ) O ( 2 ) or hydroperoxide generation in RBL 2H3 cells , and carrageenan-induced paw oedema in rats .
	manualset3
94838	1	400622	13	NULL	NULL	0	NULL	immunotherapy group 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the immunotherapy group , we also registered a negative correlation between concentrations of Dpt-specific serum IgE and IgG antibodies ( p = -0.83 ; p & lt ; 0.05 ) , at the end of the second month .
	manualset3
94839	2	400622	13	NULL	NULL	0	NULL	negative correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In the immunotherapy group , we also registered a negative correlation between concentrations of Dpt-specific serum IgE and IgG antibodies ( p = -0.83 ; p & lt ; 0.05 ) , at the end of the second month .
	manualset3
94840	3	400622	13	NULL	NULL	0	NULL	concentrations 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the immunotherapy group , we also registered a negative correlation between concentrations of Dpt-specific serum IgE and IgG antibodies ( p = -0.83 ; p & lt ; 0.05 ) , at the end of the second month .
	manualset3
94841	4	400622	13	NULL	NULL	0	NULL	Dpt-specific serum IgE antibodies 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the immunotherapy group , we also registered a negative correlation between concentrations of Dpt-specific serum IgE and IgG antibodies ( p = -0.83 ; p & lt ; 0.05 ) , at the end of the second month .
	manualset3
94842	5	400622	13	NULL	NULL	0	NULL	Dpt-specific serum IgG antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the immunotherapy group , we also registered a negative correlation between concentrations of Dpt-specific serum IgE and IgG antibodies ( p = -0.83 ; p & lt ; 0.05 ) , at the end of the second month .
	manualset3
94843	6	400622	13	NULL	NULL	0	NULL	p = -0.83 ; p & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the immunotherapy group , we also registered a negative correlation between concentrations of Dpt-specific serum IgE and IgG antibodies ( p = -0.83 ; p & lt ; 0.05 ) , at the end of the second month .
	manualset3
94844	7	400622	13	NULL	NULL	0	NULL	second month	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In the immunotherapy group , we also registered a negative correlation between concentrations of Dpt-specific serum IgE and IgG antibodies ( p = -0.83 ; p & lt ; 0.05 ) , at the end of the second month .
	manualset3
94845	1	400623	13	NULL	NULL	0	NULL	in vitro experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the in vitro experiments , we found that YC-1 significantly inhibited MDA-MB-468 cell proliferation in normoxia and hypoxia .
	manualset3
94846	2	400623	13	NULL	NULL	0	NULL	YC-1	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the in vitro experiments , we found that YC-1 significantly inhibited MDA-MB-468 cell proliferation in normoxia and hypoxia .
	manualset3
94847	3	400623	13	NULL	NULL	0	NULL	MDA-MB-468 cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the in vitro experiments , we found that YC-1 significantly inhibited MDA-MB-468 cell proliferation in normoxia and hypoxia .
	manualset3
94848	4	400623	13	NULL	NULL	0	NULL	proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the in vitro experiments , we found that YC-1 significantly inhibited MDA-MB-468 cell proliferation in normoxia and hypoxia .
	manualset3
94849	5	400623	13	NULL	NULL	0	NULL	 normoxia	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In the in vitro experiments , we found that YC-1 significantly inhibited MDA-MB-468 cell proliferation in normoxia and hypoxia .
	manualset3
94850	6	400623	13	NULL	NULL	0	NULL	hypoxia	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In the in vitro experiments , we found that YC-1 significantly inhibited MDA-MB-468 cell proliferation in normoxia and hypoxia .
	manualset3
94851	1	400624	13	NULL	NULL	0	NULL	individual patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In the individual patient , day-to-day variability of TEE may be large .
	manualset3
94852	2	400624	13	NULL	NULL	0	NULL	day-to-day variability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the individual patient , day-to-day variability of TEE may be large .
	manualset3
94853	3	400624	13	NULL	NULL	NULL	NULL	TEE	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the individual patient , day-to-day variability of TEE may be large .
	manualset3
94854	1	400625	13	NULL	NULL	0	NULL	initial experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the initial experiments , cocaine-induced locomotor activity was assessed after either acute or chronic injections of the kappa receptor agonist U-50 , 488 ( 5 mg/kg , SC ) .
	manualset3
94855	2	400625	13	NULL	NULL	0	NULL	cocaine-induced locomotor activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the initial experiments , cocaine-induced locomotor activity was assessed after either acute or chronic injections of the kappa receptor agonist U-50 , 488 ( 5 mg/kg , SC ) .
	manualset3
94856	3	400625	13	NULL	NULL	0	NULL	acute injections	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the initial experiments , cocaine-induced locomotor activity was assessed after either acute or chronic injections of the kappa receptor agonist U-50 , 488 ( 5 mg/kg , SC ) .
	manualset3
94857	4	400625	13	NULL	NULL	0	NULL	chronic injections	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the initial experiments , cocaine-induced locomotor activity was assessed after either acute or chronic injections of the kappa receptor agonist U-50 , 488 ( 5 mg/kg , SC ) .
	manualset3
94858	5	400625	13	NULL	NULL	0	NULL	kappa receptor agonist U-50	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the initial experiments , cocaine-induced locomotor activity was assessed after either acute or chronic injections of the kappa receptor agonist U-50 , 488 ( 5 mg/kg , SC ) .
	manualset3
94859	6	400625	13	NULL	NULL	0	NULL	488 ( 5 mg/kg , SC ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the initial experiments , cocaine-induced locomotor activity was assessed after either acute or chronic injections of the kappa receptor agonist U-50 , 488 ( 5 mg/kg , SC ) .
	manualset3
94860	1	400626	13	NULL	NULL	0	NULL	 initial test	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the initial test , the elevated basal levels of PRL , 61.9 + / - 9.8 ng/ml ( Mean + / - SE ) exhibited a slight but insignificant net increase ( 7.7 + / - 2.1 ng/ml ) after TRH injection in the euthyroid group .
	manualset3
94861	2	400626	13	NULL	NULL	0	NULL	basal levels of PRL	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the initial test , the elevated basal levels of PRL , 61.9 + / - 9.8 ng/ml ( Mean + / - SE ) exhibited a slight but insignificant net increase ( 7.7 + / - 2.1 ng/ml ) after TRH injection in the euthyroid group .
	manualset3
94862	3	400626	13	NULL	NULL	0	NULL	61.9 + / - 9.8 ng/ml ( Mean + / - SE )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the initial test , the elevated basal levels of PRL , 61.9 + / - 9.8 ng/ml ( Mean + / - SE ) exhibited a slight but insignificant net increase ( 7.7 + / - 2.1 ng/ml ) after TRH injection in the euthyroid group .
	manualset3
94863	4	400626	13	NULL	NULL	0	NULL	insignificant net increase ( 7.7 + / - 2.1 ng/ml )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the initial test , the elevated basal levels of PRL , 61.9 + / - 9.8 ng/ml ( Mean + / - SE ) exhibited a slight but insignificant net increase ( 7.7 + / - 2.1 ng/ml ) after TRH injection in the euthyroid group .
	manualset3
94864	5	400626	13	NULL	NULL	0	NULL	TRH injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the initial test , the elevated basal levels of PRL , 61.9 + / - 9.8 ng/ml ( Mean + / - SE ) exhibited a slight but insignificant net increase ( 7.7 + / - 2.1 ng/ml ) after TRH injection in the euthyroid group .
	manualset3
94865	6	400626	13	NULL	NULL	0	NULL	euthyroid group 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the initial test , the elevated basal levels of PRL , 61.9 + / - 9.8 ng/ml ( Mean + / - SE ) exhibited a slight but insignificant net increase ( 7.7 + / - 2.1 ng/ml ) after TRH injection in the euthyroid group .
	manualset3
94866	1	400627	13	NULL	NULL	0	NULL	insulin group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the insulin group , however , the functional recovery was barely affected by BAY o 1248 .
	manualset3
94867	2	400627	13	NULL	NULL	0	NULL	functional recovery 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the insulin group , however , the functional recovery was barely affected by BAY o 1248 .
	manualset3
94868	3	400627	13	NULL	NULL	0	NULL	BAY o 1248	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the insulin group , however , the functional recovery was barely affected by BAY o 1248 .
	manualset3
94869	1	400628	13	NULL	NULL	0	NULL	intervention group 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the intervention group the breastfed infants had the lowest incidence of allergic symptoms , followed by the infants fed the hydrolysed formula ( ns ) .
	manualset3
94870	2	400628	13	NULL	NULL	NULL	NULL	infants	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the intervention group the breastfed infants had the lowest incidence of allergic symptoms , followed by the infants fed the hydrolysed formula ( ns ) .
	manualset3
94871	3	400628	13	NULL	NULL	0	NULL	lowest incidence of allergic symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the intervention group the breastfed infants had the lowest incidence of allergic symptoms , followed by the infants fed the hydrolysed formula ( ns ) .
	manualset3
94872	4	400628	13	NULL	NULL	0	NULL	infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the intervention group the breastfed infants had the lowest incidence of allergic symptoms , followed by the infants fed the hydrolysed formula ( ns ) .
	manualset3
94873	5	400628	13	NULL	NULL	NULL	NULL	hydrolysed formula ( ns ) 	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the intervention group the breastfed infants had the lowest incidence of allergic symptoms , followed by the infants fed the hydrolysed formula ( ns ) .
	manualset3
94874	1	400629	13	NULL	NULL	0	NULL	last 20 years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last 20 years the vision of few has become a reality of collaboration of several hundred centers around the world in pediatric rheumatology research .
	manualset3
94875	2	400629	13	NULL	NULL	0	NULL	vision	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last 20 years the vision of few has become a reality of collaboration of several hundred centers around the world in pediatric rheumatology research .
	manualset3
94876	3	400629	13	NULL	NULL	0	NULL	reality	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last 20 years the vision of few has become a reality of collaboration of several hundred centers around the world in pediatric rheumatology research .
	manualset3
94877	4	400629	13	NULL	NULL	0	NULL	 collaboration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last 20 years the vision of few has become a reality of collaboration of several hundred centers around the world in pediatric rheumatology research .
	manualset3
94878	5	400629	13	NULL	NULL	0	NULL	several hundred centers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last 20 years the vision of few has become a reality of collaboration of several hundred centers around the world in pediatric rheumatology research .
	manualset3
94879	6	400629	13	NULL	NULL	0	NULL	 world	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last 20 years the vision of few has become a reality of collaboration of several hundred centers around the world in pediatric rheumatology research .
	manualset3
94880	7	400629	13	NULL	NULL	0	NULL	pediatric rheumatology research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last 20 years the vision of few has become a reality of collaboration of several hundred centers around the world in pediatric rheumatology research .
	manualset3
94881	1	400630	13	NULL	NULL	0	NULL	last decade	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last decade , hearing research has benefited tremendously from the progress of the human and mouse genome projects , as amply illustrated by the identification of many deafness genes in both human and mouse .
	manualset3
94882	2	400630	13	NULL	NULL	0	NULL	hearing research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last decade , hearing research has benefited tremendously from the progress of the human and mouse genome projects , as amply illustrated by the identification of many deafness genes in both human and mouse .
	manualset3
94883	3	400630	13	NULL	NULL	0	NULL	progress	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last decade , hearing research has benefited tremendously from the progress of the human and mouse genome projects , as amply illustrated by the identification of many deafness genes in both human and mouse .
	manualset3
94884	4	400630	13	NULL	NULL	0	NULL	human genome projects	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last decade , hearing research has benefited tremendously from the progress of the human and mouse genome projects , as amply illustrated by the identification of many deafness genes in both human and mouse .
	manualset3
94885	5	400630	13	NULL	NULL	0	NULL	mouse genome projects	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last decade , hearing research has benefited tremendously from the progress of the human and mouse genome projects , as amply illustrated by the identification of many deafness genes in both human and mouse .
	manualset3
94886	6	400630	13	NULL	NULL	0	NULL	identification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last decade , hearing research has benefited tremendously from the progress of the human and mouse genome projects , as amply illustrated by the identification of many deafness genes in both human and mouse .
	manualset3
94887	7	400630	13	NULL	NULL	0	NULL	deafness genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last decade , hearing research has benefited tremendously from the progress of the human and mouse genome projects , as amply illustrated by the identification of many deafness genes in both human and mouse .
	manualset3
94888	8	400630	13	NULL	NULL	0	NULL	 human 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last decade , hearing research has benefited tremendously from the progress of the human and mouse genome projects , as amply illustrated by the identification of many deafness genes in both human and mouse .
	manualset3
94889	9	400630	13	NULL	NULL	0	NULL	mouse	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last decade , hearing research has benefited tremendously from the progress of the human and mouse genome projects , as amply illustrated by the identification of many deafness genes in both human and mouse .
	manualset3
94890	1	400631	13	NULL	NULL	0	NULL	last decade	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last decade , target antigens have been identified and cloned , and a number of vaccine trials undertaken in both humans and laboratory animals .
	manualset3
94891	2	400631	13	NULL	NULL	0	NULL	target antigens 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last decade , target antigens have been identified and cloned , and a number of vaccine trials undertaken in both humans and laboratory animals .
	manualset3
94892	3	400631	13	NULL	NULL	0	NULL	number of vaccine trials	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last decade , target antigens have been identified and cloned , and a number of vaccine trials undertaken in both humans and laboratory animals .
	manualset3
94893	4	400631	13	NULL	NULL	NULL	NULL	humans	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the last decade , target antigens have been identified and cloned , and a number of vaccine trials undertaken in both humans and laboratory animals .
	manualset3
94894	5	400631	13	NULL	NULL	0	NULL	laboratory animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last decade , target antigens have been identified and cloned , and a number of vaccine trials undertaken in both humans and laboratory animals .
	manualset3
94895	1	400632	13	NULL	NULL	0	NULL	1 alpha ( OH ) D3 glucoside 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	1 alpha ( OH ) D3 glucoside has about 10 % activity of the free 1 alpha ( OH ) D3 , while 1 alpha ( OH ) D3 cellobioside is without any activity in chickens .
	manualset3
94896	2	400632	13	NULL	NULL	0	NULL	10 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	1 alpha ( OH ) D3 glucoside has about 10 % activity of the free 1 alpha ( OH ) D3 , while 1 alpha ( OH ) D3 cellobioside is without any activity in chickens .
	manualset3
94897	3	400632	13	NULL	NULL	0	NULL	activity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	1 alpha ( OH ) D3 glucoside has about 10 % activity of the free 1 alpha ( OH ) D3 , while 1 alpha ( OH ) D3 cellobioside is without any activity in chickens .
	manualset3
94898	4	400632	13	NULL	NULL	0	NULL	1 alpha ( OH ) D3	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	1 alpha ( OH ) D3 glucoside has about 10 % activity of the free 1 alpha ( OH ) D3 , while 1 alpha ( OH ) D3 cellobioside is without any activity in chickens .
	manualset3
94899	5	400632	13	NULL	NULL	0	NULL	1 alpha ( OH ) D3 cellobioside	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	1 alpha ( OH ) D3 glucoside has about 10 % activity of the free 1 alpha ( OH ) D3 , while 1 alpha ( OH ) D3 cellobioside is without any activity in chickens .
	manualset3
94900	6	400632	13	NULL	NULL	0	NULL	activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	1 alpha ( OH ) D3 glucoside has about 10 % activity of the free 1 alpha ( OH ) D3 , while 1 alpha ( OH ) D3 cellobioside is without any activity in chickens .
	manualset3
94901	7	400632	13	NULL	NULL	0	NULL	chickens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	1 alpha ( OH ) D3 glucoside has about 10 % activity of the free 1 alpha ( OH ) D3 , while 1 alpha ( OH ) D3 cellobioside is without any activity in chickens .
	manualset3
94902	1	400633	13	NULL	NULL	0	NULL	 last decade	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last decade , the electromorphic phenotype corresponding to extremely polymorphic zones of DNA , that include variable number of tandem repeat loci ( VNTR ) of oligonucleotide sequences , have been added to classical markers to elucidate the problems of parenthood identification and ascription in human beings .
	manualset3
94903	2	400633	13	NULL	NULL	0	NULL	electromorphic phenotype	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last decade , the electromorphic phenotype corresponding to extremely polymorphic zones of DNA , that include variable number of tandem repeat loci ( VNTR ) of oligonucleotide sequences , have been added to classical markers to elucidate the problems of parenthood identification and ascription in human beings .
	manualset3
94904	3	400633	13	NULL	NULL	0	NULL	polymorphic zones of DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last decade , the electromorphic phenotype corresponding to extremely polymorphic zones of DNA , that include variable number of tandem repeat loci ( VNTR ) of oligonucleotide sequences , have been added to classical markers to elucidate the problems of parenthood identification and ascription in human beings .
	manualset3
94905	4	400633	13	NULL	NULL	0	NULL	 variable number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last decade , the electromorphic phenotype corresponding to extremely polymorphic zones of DNA , that include variable number of tandem repeat loci ( VNTR ) of oligonucleotide sequences , have been added to classical markers to elucidate the problems of parenthood identification and ascription in human beings .
	manualset3
94906	5	400633	13	NULL	NULL	0	NULL	tandem repeat loci ( VNTR ) of oligonucleotide sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last decade , the electromorphic phenotype corresponding to extremely polymorphic zones of DNA , that include variable number of tandem repeat loci ( VNTR ) of oligonucleotide sequences , have been added to classical markers to elucidate the problems of parenthood identification and ascription in human beings .
	manualset3
94907	6	400633	13	NULL	NULL	0	NULL	classical markers 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last decade , the electromorphic phenotype corresponding to extremely polymorphic zones of DNA , that include variable number of tandem repeat loci ( VNTR ) of oligonucleotide sequences , have been added to classical markers to elucidate the problems of parenthood identification and ascription in human beings .
	manualset3
94908	7	400633	13	NULL	NULL	NULL	NULL	problems of parenthood identification	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the last decade , the electromorphic phenotype corresponding to extremely polymorphic zones of DNA , that include variable number of tandem repeat loci ( VNTR ) of oligonucleotide sequences , have been added to classical markers to elucidate the problems of parenthood identification and ascription in human beings .
	manualset3
94909	8	400633	13	NULL	NULL	NULL	NULL	problems of parenthood ascription 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the last decade , the electromorphic phenotype corresponding to extremely polymorphic zones of DNA , that include variable number of tandem repeat loci ( VNTR ) of oligonucleotide sequences , have been added to classical markers to elucidate the problems of parenthood identification and ascription in human beings .
	manualset3
94911	10	400633	13	NULL	NULL	0	NULL	human beings	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last decade , the electromorphic phenotype corresponding to extremely polymorphic zones of DNA , that include variable number of tandem repeat loci ( VNTR ) of oligonucleotide sequences , have been added to classical markers to elucidate the problems of parenthood identification and ascription in human beings .
	manualset3
94912	1	400634	13	NULL	NULL	0	NULL	last decade 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last decade considerable understanding of the biochemical process within plants has been developed .
	manualset3
94913	2	400634	13	NULL	NULL	0	NULL	understanding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last decade considerable understanding of the biochemical process within plants has been developed .
	manualset3
94914	3	400634	13	NULL	NULL	0	NULL	biochemical process	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last decade considerable understanding of the biochemical process within plants has been developed .
	manualset3
94915	4	400634	13	NULL	NULL	0	NULL	 plants 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last decade considerable understanding of the biochemical process within plants has been developed .
	manualset3
94916	1	400635	13	NULL	NULL	0	NULL	 last few years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last few years a number of studies based on isoenzyme overexpression indicated that the PKC family coordinates a complex network of pivotal signal transduction pathways and pathway crosstalks , which regulate cell growth and differentiation , neoplastic transformation and malignant progression .
	manualset3
94917	2	400635	13	NULL	NULL	0	NULL	number of studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last few years a number of studies based on isoenzyme overexpression indicated that the PKC family coordinates a complex network of pivotal signal transduction pathways and pathway crosstalks , which regulate cell growth and differentiation , neoplastic transformation and malignant progression .
	manualset3
94918	3	400635	13	NULL	NULL	0	NULL	 isoenzyme overexpression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last few years a number of studies based on isoenzyme overexpression indicated that the PKC family coordinates a complex network of pivotal signal transduction pathways and pathway crosstalks , which regulate cell growth and differentiation , neoplastic transformation and malignant progression .
	manualset3
94919	4	400635	13	NULL	NULL	0	NULL	PKC family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last few years a number of studies based on isoenzyme overexpression indicated that the PKC family coordinates a complex network of pivotal signal transduction pathways and pathway crosstalks , which regulate cell growth and differentiation , neoplastic transformation and malignant progression .
	manualset3
94920	5	400635	13	NULL	NULL	NULL	NULL	complex network	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the last few years a number of studies based on isoenzyme overexpression indicated that the PKC family coordinates a complex network of pivotal signal transduction pathways and pathway crosstalks , which regulate cell growth and differentiation , neoplastic transformation and malignant progression .
	manualset3
94921	6	400635	13	NULL	NULL	0	NULL	pivotal signal transduction pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last few years a number of studies based on isoenzyme overexpression indicated that the PKC family coordinates a complex network of pivotal signal transduction pathways and pathway crosstalks , which regulate cell growth and differentiation , neoplastic transformation and malignant progression .
	manualset3
94922	7	400635	13	NULL	NULL	0	NULL	pathway crosstalks 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last few years a number of studies based on isoenzyme overexpression indicated that the PKC family coordinates a complex network of pivotal signal transduction pathways and pathway crosstalks , which regulate cell growth and differentiation , neoplastic transformation and malignant progression .
	manualset3
94923	8	400635	13	NULL	NULL	0	NULL	cell growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last few years a number of studies based on isoenzyme overexpression indicated that the PKC family coordinates a complex network of pivotal signal transduction pathways and pathway crosstalks , which regulate cell growth and differentiation , neoplastic transformation and malignant progression .
	manualset3
94924	9	400635	13	NULL	NULL	0	NULL	differentiation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last few years a number of studies based on isoenzyme overexpression indicated that the PKC family coordinates a complex network of pivotal signal transduction pathways and pathway crosstalks , which regulate cell growth and differentiation , neoplastic transformation and malignant progression .
	manualset3
94925	10	400635	13	NULL	NULL	0	NULL	neoplastic transformation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last few years a number of studies based on isoenzyme overexpression indicated that the PKC family coordinates a complex network of pivotal signal transduction pathways and pathway crosstalks , which regulate cell growth and differentiation , neoplastic transformation and malignant progression .
	manualset3
94926	11	400635	13	NULL	NULL	0	NULL	malignant progression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last few years a number of studies based on isoenzyme overexpression indicated that the PKC family coordinates a complex network of pivotal signal transduction pathways and pathway crosstalks , which regulate cell growth and differentiation , neoplastic transformation and malignant progression .
	manualset3
94927	1	400636	13	NULL	NULL	0	NULL	last few years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last few years we have witnessed a reorientation process in the diagnosis and treatment of cancer , and advances in cancer research point to the need for selective or specific immunomodulation therapies .
	manualset3
94928	2	400636	13	NULL	NULL	0	NULL	reorientation process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last few years we have witnessed a reorientation process in the diagnosis and treatment of cancer , and advances in cancer research point to the need for selective or specific immunomodulation therapies .
	manualset3
94929	3	400636	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last few years we have witnessed a reorientation process in the diagnosis and treatment of cancer , and advances in cancer research point to the need for selective or specific immunomodulation therapies .
	manualset3
94930	4	400636	13	NULL	NULL	0	NULL	 treatment of cancer	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last few years we have witnessed a reorientation process in the diagnosis and treatment of cancer , and advances in cancer research point to the need for selective or specific immunomodulation therapies .
	manualset3
94931	5	400636	13	NULL	NULL	0	NULL	advances	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last few years we have witnessed a reorientation process in the diagnosis and treatment of cancer , and advances in cancer research point to the need for selective or specific immunomodulation therapies .
	manualset3
94932	6	400636	13	NULL	NULL	NULL	NULL	cancer research	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the last few years we have witnessed a reorientation process in the diagnosis and treatment of cancer , and advances in cancer research point to the need for selective or specific immunomodulation therapies .
	manualset3
94933	7	400636	13	NULL	NULL	0	NULL	need	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last few years we have witnessed a reorientation process in the diagnosis and treatment of cancer , and advances in cancer research point to the need for selective or specific immunomodulation therapies .
	manualset3
94934	8	400636	13	NULL	NULL	0	NULL	selective immunomodulation therapies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last few years we have witnessed a reorientation process in the diagnosis and treatment of cancer , and advances in cancer research point to the need for selective or specific immunomodulation therapies .
	manualset3
94935	9	400636	13	NULL	NULL	0	NULL	specific immunomodulation therapies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the last few years we have witnessed a reorientation process in the diagnosis and treatment of cancer , and advances in cancer research point to the need for selective or specific immunomodulation therapies .
	manualset3
94936	1	400637	13	NULL	NULL	0	NULL	case	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In the latter case , the number of invading organisms determines whether induction of a virulence gene is necessary for successful infection .
	manualset3
94937	2	400637	13	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the latter case , the number of invading organisms determines whether induction of a virulence gene is necessary for successful infection .
	manualset3
94938	3	400637	13	NULL	NULL	0	NULL	organisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the latter case , the number of invading organisms determines whether induction of a virulence gene is necessary for successful infection .
	manualset3
94939	4	400637	13	NULL	NULL	0	NULL	 induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the latter case , the number of invading organisms determines whether induction of a virulence gene is necessary for successful infection .
	manualset3
94940	5	400637	13	NULL	NULL	0	NULL	virulence gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In the latter case , the number of invading organisms determines whether induction of a virulence gene is necessary for successful infection .
	manualset3
94941	6	400637	13	NULL	NULL	0	NULL	successful infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the latter case , the number of invading organisms determines whether induction of a virulence gene is necessary for successful infection .
	manualset3
94942	1	400638	13	NULL	NULL	0	NULL	latter case	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the latter case , the threshold between zone 1 and zone 2 may be around 100-200 m and , perhaps , may have been evolutionary determined by the natural human high resolution visual range , which characterizes an area of interest where the benefits are assumed to be randomly and uniformly distributed .
	manualset3
94943	2	400638	13	NULL	NULL	0	NULL	threshold between zone 1 and zone 2 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the latter case , the threshold between zone 1 and zone 2 may be around 100-200 m and , perhaps , may have been evolutionary determined by the natural human high resolution visual range , which characterizes an area of interest where the benefits are assumed to be randomly and uniformly distributed .
	manualset3
94944	3	400638	13	NULL	NULL	0	NULL	100-200 m	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the latter case , the threshold between zone 1 and zone 2 may be around 100-200 m and , perhaps , may have been evolutionary determined by the natural human high resolution visual range , which characterizes an area of interest where the benefits are assumed to be randomly and uniformly distributed .
	manualset3
94945	4	400638	13	NULL	NULL	0	NULL	natural human high resolution visual range 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the latter case , the threshold between zone 1 and zone 2 may be around 100-200 m and , perhaps , may have been evolutionary determined by the natural human high resolution visual range , which characterizes an area of interest where the benefits are assumed to be randomly and uniformly distributed .
	manualset3
94946	5	400638	13	NULL	NULL	0	NULL	area of interest	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the latter case , the threshold between zone 1 and zone 2 may be around 100-200 m and , perhaps , may have been evolutionary determined by the natural human high resolution visual range , which characterizes an area of interest where the benefits are assumed to be randomly and uniformly distributed .
	manualset3
94947	6	400638	13	NULL	NULL	0	NULL	benefits	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the latter case , the threshold between zone 1 and zone 2 may be around 100-200 m and , perhaps , may have been evolutionary determined by the natural human high resolution visual range , which characterizes an area of interest where the benefits are assumed to be randomly and uniformly distributed .
	manualset3
94948	1	400639	13	NULL	NULL	0	NULL	 light of other findings	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the light of other findings from the larger study , we think it likely that the negative associations between language measures and MEE reflect confounding factors that contribute , on the one hand , to the duration of OM in young children and , on the other hand , to slow development of their language skills .
	manualset3
94949	2	400639	13	NULL	NULL	0	NULL	larger study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the light of other findings from the larger study , we think it likely that the negative associations between language measures and MEE reflect confounding factors that contribute , on the one hand , to the duration of OM in young children and , on the other hand , to slow development of their language skills .
	manualset3
94950	3	400639	13	NULL	NULL	NULL	NULL	negative associations	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the light of other findings from the larger study , we think it likely that the negative associations between language measures and MEE reflect confounding factors that contribute , on the one hand , to the duration of OM in young children and , on the other hand , to slow development of their language skills .
	manualset3
94951	4	400639	13	NULL	NULL	NULL	NULL	language measures	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the light of other findings from the larger study , we think it likely that the negative associations between language measures and MEE reflect confounding factors that contribute , on the one hand , to the duration of OM in young children and , on the other hand , to slow development of their language skills .
	manualset3
94952	5	400639	13	NULL	NULL	0	NULL	MEE reflect 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the light of other findings from the larger study , we think it likely that the negative associations between language measures and MEE reflect confounding factors that contribute , on the one hand , to the duration of OM in young children and , on the other hand , to slow development of their language skills .
	manualset3
94953	6	400639	13	NULL	NULL	0	NULL	factors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the light of other findings from the larger study , we think it likely that the negative associations between language measures and MEE reflect confounding factors that contribute , on the one hand , to the duration of OM in young children and , on the other hand , to slow development of their language skills .
	manualset3
94954	7	400639	13	NULL	NULL	0	NULL	hand	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the light of other findings from the larger study , we think it likely that the negative associations between language measures and MEE reflect confounding factors that contribute , on the one hand , to the duration of OM in young children and , on the other hand , to slow development of their language skills .
	manualset3
94955	8	400639	13	NULL	NULL	0	NULL	duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the light of other findings from the larger study , we think it likely that the negative associations between language measures and MEE reflect confounding factors that contribute , on the one hand , to the duration of OM in young children and , on the other hand , to slow development of their language skills .
	manualset3
94956	9	400639	13	NULL	NULL	0	NULL	OM	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the light of other findings from the larger study , we think it likely that the negative associations between language measures and MEE reflect confounding factors that contribute , on the one hand , to the duration of OM in young children and , on the other hand , to slow development of their language skills .
	manualset3
94957	10	400639	13	NULL	NULL	0	NULL	young children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the light of other findings from the larger study , we think it likely that the negative associations between language measures and MEE reflect confounding factors that contribute , on the one hand , to the duration of OM in young children and , on the other hand , to slow development of their language skills .
	manualset3
94958	11	400639	13	NULL	NULL	0	NULL	hand	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the light of other findings from the larger study , we think it likely that the negative associations between language measures and MEE reflect confounding factors that contribute , on the one hand , to the duration of OM in young children and , on the other hand , to slow development of their language skills .
	manualset3
94959	12	400639	13	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the light of other findings from the larger study , we think it likely that the negative associations between language measures and MEE reflect confounding factors that contribute , on the one hand , to the duration of OM in young children and , on the other hand , to slow development of their language skills .
	manualset3
94960	13	400639	13	NULL	NULL	0	NULL	language skills	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the light of other findings from the larger study , we think it likely that the negative associations between language measures and MEE reflect confounding factors that contribute , on the one hand , to the duration of OM in young children and , on the other hand , to slow development of their language skills .
	manualset3
94961	1	400640	13	NULL	NULL	0	NULL	literature 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the literature , it is well reported that this inhibitor can determine serious cardiovascular side effects , including congestive heart failure , arrhythmia and acute coronary syndrome .
	manualset3
94962	2	400640	13	NULL	NULL	0	NULL	inhibitor 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the literature , it is well reported that this inhibitor can determine serious cardiovascular side effects , including congestive heart failure , arrhythmia and acute coronary syndrome .
	manualset3
94963	3	400640	13	NULL	NULL	0	NULL	serious cardiovascular side effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the literature , it is well reported that this inhibitor can determine serious cardiovascular side effects , including congestive heart failure , arrhythmia and acute coronary syndrome .
	manualset3
94964	4	400640	13	NULL	NULL	0	NULL	congestive heart failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the literature , it is well reported that this inhibitor can determine serious cardiovascular side effects , including congestive heart failure , arrhythmia and acute coronary syndrome .
	manualset3
94965	5	400640	13	NULL	NULL	0	NULL	arrhythmia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the literature , it is well reported that this inhibitor can determine serious cardiovascular side effects , including congestive heart failure , arrhythmia and acute coronary syndrome .
	manualset3
94966	6	400640	13	NULL	NULL	0	NULL	acute coronary syndrome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the literature , it is well reported that this inhibitor can determine serious cardiovascular side effects , including congestive heart failure , arrhythmia and acute coronary syndrome .
	manualset3
94967	1	400641	13	NULL	NULL	0	NULL	logistic regression analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the logistic regression analysis of gene-gene interaction , we found a significant interaction effect of rs7525948 of DLGAP3 and rs2228622 of SLC1A1 ( permutation P = 0.036 ) on AAP-induced OC symptoms , with a 30.2 times higher odds for individuals carrying risk genotypes at both loci in comparison with the reference group , which had no risk genotypes .
	manualset3
94968	2	400641	13	NULL	NULL	0	NULL	gene-gene interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the logistic regression analysis of gene-gene interaction , we found a significant interaction effect of rs7525948 of DLGAP3 and rs2228622 of SLC1A1 ( permutation P = 0.036 ) on AAP-induced OC symptoms , with a 30.2 times higher odds for individuals carrying risk genotypes at both loci in comparison with the reference group , which had no risk genotypes .
	manualset3
94969	3	400641	13	NULL	NULL	0	NULL	interaction effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the logistic regression analysis of gene-gene interaction , we found a significant interaction effect of rs7525948 of DLGAP3 and rs2228622 of SLC1A1 ( permutation P = 0.036 ) on AAP-induced OC symptoms , with a 30.2 times higher odds for individuals carrying risk genotypes at both loci in comparison with the reference group , which had no risk genotypes .
	manualset3
94970	4	400641	13	NULL	NULL	0	NULL	rs7525948 of DLGAP3	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the logistic regression analysis of gene-gene interaction , we found a significant interaction effect of rs7525948 of DLGAP3 and rs2228622 of SLC1A1 ( permutation P = 0.036 ) on AAP-induced OC symptoms , with a 30.2 times higher odds for individuals carrying risk genotypes at both loci in comparison with the reference group , which had no risk genotypes .
	manualset3
94971	5	400641	13	NULL	NULL	0	NULL	rs2228622 of SLC1A1 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the logistic regression analysis of gene-gene interaction , we found a significant interaction effect of rs7525948 of DLGAP3 and rs2228622 of SLC1A1 ( permutation P = 0.036 ) on AAP-induced OC symptoms , with a 30.2 times higher odds for individuals carrying risk genotypes at both loci in comparison with the reference group , which had no risk genotypes .
	manualset3
94972	6	400641	13	NULL	NULL	0	NULL	permutation P = 0.036	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the logistic regression analysis of gene-gene interaction , we found a significant interaction effect of rs7525948 of DLGAP3 and rs2228622 of SLC1A1 ( permutation P = 0.036 ) on AAP-induced OC symptoms , with a 30.2 times higher odds for individuals carrying risk genotypes at both loci in comparison with the reference group , which had no risk genotypes .
	manualset3
94973	7	400641	13	NULL	NULL	0	NULL	AAP-induced OC symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the logistic regression analysis of gene-gene interaction , we found a significant interaction effect of rs7525948 of DLGAP3 and rs2228622 of SLC1A1 ( permutation P = 0.036 ) on AAP-induced OC symptoms , with a 30.2 times higher odds for individuals carrying risk genotypes at both loci in comparison with the reference group , which had no risk genotypes .
	manualset3
94974	8	400641	13	NULL	NULL	0	NULL	30.2 times higher odds 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the logistic regression analysis of gene-gene interaction , we found a significant interaction effect of rs7525948 of DLGAP3 and rs2228622 of SLC1A1 ( permutation P = 0.036 ) on AAP-induced OC symptoms , with a 30.2 times higher odds for individuals carrying risk genotypes at both loci in comparison with the reference group , which had no risk genotypes .
	manualset3
94975	9	400641	13	NULL	NULL	0	NULL	 individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the logistic regression analysis of gene-gene interaction , we found a significant interaction effect of rs7525948 of DLGAP3 and rs2228622 of SLC1A1 ( permutation P = 0.036 ) on AAP-induced OC symptoms , with a 30.2 times higher odds for individuals carrying risk genotypes at both loci in comparison with the reference group , which had no risk genotypes .
	manualset3
94976	10	400641	13	NULL	NULL	0	NULL	risk genotypes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the logistic regression analysis of gene-gene interaction , we found a significant interaction effect of rs7525948 of DLGAP3 and rs2228622 of SLC1A1 ( permutation P = 0.036 ) on AAP-induced OC symptoms , with a 30.2 times higher odds for individuals carrying risk genotypes at both loci in comparison with the reference group , which had no risk genotypes .
	manualset3
94977	11	400641	13	NULL	NULL	0	NULL	loci	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the logistic regression analysis of gene-gene interaction , we found a significant interaction effect of rs7525948 of DLGAP3 and rs2228622 of SLC1A1 ( permutation P = 0.036 ) on AAP-induced OC symptoms , with a 30.2 times higher odds for individuals carrying risk genotypes at both loci in comparison with the reference group , which had no risk genotypes .
	manualset3
94978	12	400641	13	NULL	NULL	0	NULL	comparison 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In the logistic regression analysis of gene-gene interaction , we found a significant interaction effect of rs7525948 of DLGAP3 and rs2228622 of SLC1A1 ( permutation P = 0.036 ) on AAP-induced OC symptoms , with a 30.2 times higher odds for individuals carrying risk genotypes at both loci in comparison with the reference group , which had no risk genotypes .
	manualset3
94979	13	400641	13	NULL	NULL	0	NULL	reference group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the logistic regression analysis of gene-gene interaction , we found a significant interaction effect of rs7525948 of DLGAP3 and rs2228622 of SLC1A1 ( permutation P = 0.036 ) on AAP-induced OC symptoms , with a 30.2 times higher odds for individuals carrying risk genotypes at both loci in comparison with the reference group , which had no risk genotypes .
	manualset3
94980	14	400641	13	NULL	NULL	0	NULL	risk genotypes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the logistic regression analysis of gene-gene interaction , we found a significant interaction effect of rs7525948 of DLGAP3 and rs2228622 of SLC1A1 ( permutation P = 0.036 ) on AAP-induced OC symptoms , with a 30.2 times higher odds for individuals carrying risk genotypes at both loci in comparison with the reference group , which had no risk genotypes .
	manualset3
94981	1	400642	13	NULL	NULL	0	NULL	long-term studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the long-term studies , the use of aripiprazole was associated with continued efficacy , good compliance and increased time-to-relapse .
	manualset3
94982	2	400642	13	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the long-term studies , the use of aripiprazole was associated with continued efficacy , good compliance and increased time-to-relapse .
	manualset3
94983	3	400642	13	NULL	NULL	0	NULL	aripiprazole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the long-term studies , the use of aripiprazole was associated with continued efficacy , good compliance and increased time-to-relapse .
	manualset3
94984	4	400642	13	NULL	NULL	0	NULL	efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the long-term studies , the use of aripiprazole was associated with continued efficacy , good compliance and increased time-to-relapse .
	manualset3
94985	5	400642	13	NULL	NULL	0	NULL	good compliance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the long-term studies , the use of aripiprazole was associated with continued efficacy , good compliance and increased time-to-relapse .
	manualset3
94986	6	400642	13	NULL	NULL	0	NULL	time-to-relapse 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In the long-term studies , the use of aripiprazole was associated with continued efficacy , good compliance and increased time-to-relapse .
	manualset3
94987	1	400643	13	NULL	NULL	0	NULL	lumen 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the lumen , the dipeptides of dietary origin apparently enter the cell through a single transport system of broad specificity in the monkey and possibly also in man .
	manualset3
94988	2	400643	13	NULL	NULL	0	NULL	dipeptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	In the lumen , the dipeptides of dietary origin apparently enter the cell through a single transport system of broad specificity in the monkey and possibly also in man .
	manualset3
94989	3	400643	13	NULL	NULL	0	NULL	dietary origin	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	In the lumen , the dipeptides of dietary origin apparently enter the cell through a single transport system of broad specificity in the monkey and possibly also in man .
	manualset3
94990	4	400643	13	NULL	NULL	0	NULL	cell 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the lumen , the dipeptides of dietary origin apparently enter the cell through a single transport system of broad specificity in the monkey and possibly also in man .
	manualset3
94991	5	400643	13	NULL	NULL	0	NULL	single transport system	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the lumen , the dipeptides of dietary origin apparently enter the cell through a single transport system of broad specificity in the monkey and possibly also in man .
	manualset3
94992	6	400643	13	NULL	NULL	NULL	NULL	broad specificity	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the lumen , the dipeptides of dietary origin apparently enter the cell through a single transport system of broad specificity in the monkey and possibly also in man .
	manualset3
94993	7	400643	13	NULL	NULL	0	NULL	monkey 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the lumen , the dipeptides of dietary origin apparently enter the cell through a single transport system of broad specificity in the monkey and possibly also in man .
	manualset3
94994	8	400643	13	NULL	NULL	0	NULL	man	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In the lumen , the dipeptides of dietary origin apparently enter the cell through a single transport system of broad specificity in the monkey and possibly also in man .
	manualset3
94995	1	400644	13	NULL	NULL	0	NULL	main study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the main study , rats were evaluated for persistent nervous system effects the week following exposure to 0 , 200 , 630 , or 2000 ppm 1 , 1 , 1-T for 6 h/day , 5 days/week , for 13 weeks .
	manualset3
94996	2	400644	13	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the main study , rats were evaluated for persistent nervous system effects the week following exposure to 0 , 200 , 630 , or 2000 ppm 1 , 1 , 1-T for 6 h/day , 5 days/week , for 13 weeks .
	manualset3
94997	3	400644	13	NULL	NULL	0	NULL	persistent nervous system effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the main study , rats were evaluated for persistent nervous system effects the week following exposure to 0 , 200 , 630 , or 2000 ppm 1 , 1 , 1-T for 6 h/day , 5 days/week , for 13 weeks .
	manualset3
94998	4	400644	13	NULL	NULL	0	NULL	week 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the main study , rats were evaluated for persistent nervous system effects the week following exposure to 0 , 200 , 630 , or 2000 ppm 1 , 1 , 1-T for 6 h/day , 5 days/week , for 13 weeks .
	manualset3
94999	5	400644	13	NULL	NULL	0	NULL	 exposure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the main study , rats were evaluated for persistent nervous system effects the week following exposure to 0 , 200 , 630 , or 2000 ppm 1 , 1 , 1-T for 6 h/day , 5 days/week , for 13 weeks .
	manualset3
95000	6	400644	13	NULL	NULL	0	NULL	0 ppm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the main study , rats were evaluated for persistent nervous system effects the week following exposure to 0 , 200 , 630 , or 2000 ppm 1 , 1 , 1-T for 6 h/day , 5 days/week , for 13 weeks .
	manualset3
95001	7	400644	13	NULL	NULL	0	NULL	200 ppm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the main study , rats were evaluated for persistent nervous system effects the week following exposure to 0 , 200 , 630 , or 2000 ppm 1 , 1 , 1-T for 6 h/day , 5 days/week , for 13 weeks .
	manualset3
95002	8	400644	13	NULL	NULL	0	NULL	 630 ppm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the main study , rats were evaluated for persistent nervous system effects the week following exposure to 0 , 200 , 630 , or 2000 ppm 1 , 1 , 1-T for 6 h/day , 5 days/week , for 13 weeks .
	manualset3
95003	9	400644	13	NULL	NULL	0	NULL	2000 ppm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the main study , rats were evaluated for persistent nervous system effects the week following exposure to 0 , 200 , 630 , or 2000 ppm 1 , 1 , 1-T for 6 h/day , 5 days/week , for 13 weeks .
	manualset3
95004	10	400644	13	NULL	NULL	0	NULL	1-T for 6 h/day	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the main study , rats were evaluated for persistent nervous system effects the week following exposure to 0 , 200 , 630 , or 2000 ppm 1 , 1 , 1-T for 6 h/day , 5 days/week , for 13 weeks .
	manualset3
95005	11	400644	13	NULL	NULL	0	NULL	1-T for 5 days/week	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the main study , rats were evaluated for persistent nervous system effects the week following exposure to 0 , 200 , 630 , or 2000 ppm 1 , 1 , 1-T for 6 h/day , 5 days/week , for 13 weeks .
	manualset3
95006	12	400644	13	NULL	NULL	0	NULL	1-T for 13 weeks	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the main study , rats were evaluated for persistent nervous system effects the week following exposure to 0 , 200 , 630 , or 2000 ppm 1 , 1 , 1-T for 6 h/day , 5 days/week , for 13 weeks .
	manualset3
95007	1	400645	13	NULL	NULL	0	NULL	majority of cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the majority of cases , locoregional treatment is curative and systemic therapy is not indicated .
	manualset3
95008	2	400645	13	NULL	NULL	0	NULL	locoregional treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the majority of cases , locoregional treatment is curative and systemic therapy is not indicated .
	manualset3
95009	3	400645	13	NULL	NULL	0	NULL	curative therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the majority of cases , locoregional treatment is curative and systemic therapy is not indicated .
	manualset3
95010	4	400645	13	NULL	NULL	0	NULL	systemic therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the majority of cases , locoregional treatment is curative and systemic therapy is not indicated .
	manualset3
95011	1	400646	13	NULL	NULL	0	NULL	majority of cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the majority of cases it is possible to ascertain the aetiology from a consideration of the clinical and serological findings , together with ordinary radiography , conventional tomography or computed tomography .
	manualset3
95012	2	400646	13	NULL	NULL	0	NULL	aetiology 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the majority of cases it is possible to ascertain the aetiology from a consideration of the clinical and serological findings , together with ordinary radiography , conventional tomography or computed tomography .
	manualset3
95013	3	400646	13	NULL	NULL	0	NULL	consideration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the majority of cases it is possible to ascertain the aetiology from a consideration of the clinical and serological findings , together with ordinary radiography , conventional tomography or computed tomography .
	manualset3
95014	4	400646	13	NULL	NULL	0	NULL	clinical findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the majority of cases it is possible to ascertain the aetiology from a consideration of the clinical and serological findings , together with ordinary radiography , conventional tomography or computed tomography .
	manualset3
95015	5	400646	13	NULL	NULL	0	NULL	serological findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the majority of cases it is possible to ascertain the aetiology from a consideration of the clinical and serological findings , together with ordinary radiography , conventional tomography or computed tomography .
	manualset3
95016	6	400646	13	NULL	NULL	0	NULL	ordinary radiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the majority of cases it is possible to ascertain the aetiology from a consideration of the clinical and serological findings , together with ordinary radiography , conventional tomography or computed tomography .
	manualset3
95017	7	400646	13	NULL	NULL	0	NULL	conventional tomography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the majority of cases it is possible to ascertain the aetiology from a consideration of the clinical and serological findings , together with ordinary radiography , conventional tomography or computed tomography .
	manualset3
95018	8	400646	13	NULL	NULL	0	NULL	computed tomography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the majority of cases it is possible to ascertain the aetiology from a consideration of the clinical and serological findings , together with ordinary radiography , conventional tomography or computed tomography .
	manualset3
95019	1	400647	13	NULL	NULL	NULL	NULL	mesopic condition	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the mesopic condition rod-dominant cells showed complex electrical membrane properties as the result of electric interaction between the above two differnt ionic mechanisms activated by rod and cone inputs .
	manualset3
95020	2	400647	13	NULL	NULL	0	NULL	rod-dominant cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mesopic condition rod-dominant cells showed complex electrical membrane properties as the result of electric interaction between the above two differnt ionic mechanisms activated by rod and cone inputs .
	manualset3
95021	3	400647	13	NULL	NULL	0	NULL	complex electrical membrane properties 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mesopic condition rod-dominant cells showed complex electrical membrane properties as the result of electric interaction between the above two differnt ionic mechanisms activated by rod and cone inputs .
	manualset3
95022	4	400647	13	NULL	NULL	0	NULL	result of electric interaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mesopic condition rod-dominant cells showed complex electrical membrane properties as the result of electric interaction between the above two differnt ionic mechanisms activated by rod and cone inputs .
	manualset3
95023	5	400647	13	NULL	NULL	0	NULL	two differnt ionic mechanisms 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mesopic condition rod-dominant cells showed complex electrical membrane properties as the result of electric interaction between the above two differnt ionic mechanisms activated by rod and cone inputs .
	manualset3
95024	6	400647	13	NULL	NULL	0	NULL	rod inputs	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mesopic condition rod-dominant cells showed complex electrical membrane properties as the result of electric interaction between the above two differnt ionic mechanisms activated by rod and cone inputs .
	manualset3
95025	7	400647	13	NULL	NULL	0	NULL	cone inputs	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mesopic condition rod-dominant cells showed complex electrical membrane properties as the result of electric interaction between the above two differnt ionic mechanisms activated by rod and cone inputs .
	manualset3
95026	1	400648	13	NULL	NULL	0	NULL	model	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In the model , the continuously changing rate of water inflow from the aquifer to the well is approximated by a step function with a finite difference time step .
	manualset3
95027	2	400648	13	NULL	NULL	0	NULL	rate of water inflow	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the model , the continuously changing rate of water inflow from the aquifer to the well is approximated by a step function with a finite difference time step .
	manualset3
95028	3	400648	13	NULL	NULL	0	NULL	aquifer	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the model , the continuously changing rate of water inflow from the aquifer to the well is approximated by a step function with a finite difference time step .
	manualset3
95029	4	400648	13	NULL	NULL	0	NULL	well 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the model , the continuously changing rate of water inflow from the aquifer to the well is approximated by a step function with a finite difference time step .
	manualset3
95030	5	400648	13	NULL	NULL	0	NULL	 step function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the model , the continuously changing rate of water inflow from the aquifer to the well is approximated by a step function with a finite difference time step .
	manualset3
95031	6	400648	13	NULL	NULL	0	NULL	difference time step	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the model , the continuously changing rate of water inflow from the aquifer to the well is approximated by a step function with a finite difference time step .
	manualset3
95032	1	400649	13	NULL	NULL	0	NULL	monkey	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the monkey , like the rat , the labeling in the dorsal raphe was light but numerous labeled neurons were present in the periaqueductal gray and the adjacent nucleus cuneiformis .
	manualset3
95033	2	400649	13	NULL	NULL	0	NULL	rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the monkey , like the rat , the labeling in the dorsal raphe was light but numerous labeled neurons were present in the periaqueductal gray and the adjacent nucleus cuneiformis .
	manualset3
95034	3	400649	13	NULL	NULL	0	NULL	labeling 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the monkey , like the rat , the labeling in the dorsal raphe was light but numerous labeled neurons were present in the periaqueductal gray and the adjacent nucleus cuneiformis .
	manualset3
95035	4	400649	13	NULL	NULL	0	NULL	dorsal raphe	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the monkey , like the rat , the labeling in the dorsal raphe was light but numerous labeled neurons were present in the periaqueductal gray and the adjacent nucleus cuneiformis .
	manualset3
95036	5	400649	13	NULL	NULL	0	NULL	 light	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the monkey , like the rat , the labeling in the dorsal raphe was light but numerous labeled neurons were present in the periaqueductal gray and the adjacent nucleus cuneiformis .
	manualset3
95037	6	400649	13	NULL	NULL	0	NULL	neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the monkey , like the rat , the labeling in the dorsal raphe was light but numerous labeled neurons were present in the periaqueductal gray and the adjacent nucleus cuneiformis .
	manualset3
95038	7	400649	13	NULL	NULL	0	NULL	periaqueductal gray	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the monkey , like the rat , the labeling in the dorsal raphe was light but numerous labeled neurons were present in the periaqueductal gray and the adjacent nucleus cuneiformis .
	manualset3
95039	8	400649	13	NULL	NULL	0	NULL	nucleus cuneiformis 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the monkey , like the rat , the labeling in the dorsal raphe was light but numerous labeled neurons were present in the periaqueductal gray and the adjacent nucleus cuneiformis .
	manualset3
95040	1	400650	13	NULL	NULL	0	NULL	syllables	Language												NULL		0	NULL	NULL	NULL	NULL	NULL	In the more stressed syllables , the tongue dorsum retracts more , likely to make a more distinct back vowel .
	manualset3
95041	2	400650	13	NULL	NULL	0	NULL	tongue dorsum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the more stressed syllables , the tongue dorsum retracts more , likely to make a more distinct back vowel .
	manualset3
95043	4	400650	13	NULL	NULL	0	NULL	vowel	Language												NULL		0	NULL	NULL	NULL	NULL	NULL	In the more stressed syllables , the tongue dorsum retracts more , likely to make a more distinct back vowel .
	manualset3
95122	1	400651	13	NULL	NULL	0	NULL	 mussels	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mussels from station C , located in the channel from the lagoon to the Mediterranean and submitted to pollutants ( urban wastes from Bizerta and hydrocarbons from the maritime traffic ) , acetylcholinesterase activities were lower than in those from station J. In conclusion , the variations in acetylcholinesterase activity observed between stations in both species may be the result of pollution and of the environmental conditions .
	manualset3
95123	2	400651	13	NULL	NULL	0	NULL	station C	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mussels from station C , located in the channel from the lagoon to the Mediterranean and submitted to pollutants ( urban wastes from Bizerta and hydrocarbons from the maritime traffic ) , acetylcholinesterase activities were lower than in those from station J. In conclusion , the variations in acetylcholinesterase activity observed between stations in both species may be the result of pollution and of the environmental conditions .
	manualset3
95124	3	400651	13	NULL	NULL	0	NULL	channel	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mussels from station C , located in the channel from the lagoon to the Mediterranean and submitted to pollutants ( urban wastes from Bizerta and hydrocarbons from the maritime traffic ) , acetylcholinesterase activities were lower than in those from station J. In conclusion , the variations in acetylcholinesterase activity observed between stations in both species may be the result of pollution and of the environmental conditions .
	manualset3
95125	4	400651	13	NULL	NULL	0	NULL	lagoon	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mussels from station C , located in the channel from the lagoon to the Mediterranean and submitted to pollutants ( urban wastes from Bizerta and hydrocarbons from the maritime traffic ) , acetylcholinesterase activities were lower than in those from station J. In conclusion , the variations in acetylcholinesterase activity observed between stations in both species may be the result of pollution and of the environmental conditions .
	manualset3
95126	5	400651	13	NULL	NULL	0	NULL	Mediterranean	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mussels from station C , located in the channel from the lagoon to the Mediterranean and submitted to pollutants ( urban wastes from Bizerta and hydrocarbons from the maritime traffic ) , acetylcholinesterase activities were lower than in those from station J. In conclusion , the variations in acetylcholinesterase activity observed between stations in both species may be the result of pollution and of the environmental conditions .
	manualset3
95127	6	400651	13	NULL	NULL	0	NULL	pollutants	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mussels from station C , located in the channel from the lagoon to the Mediterranean and submitted to pollutants ( urban wastes from Bizerta and hydrocarbons from the maritime traffic ) , acetylcholinesterase activities were lower than in those from station J. In conclusion , the variations in acetylcholinesterase activity observed between stations in both species may be the result of pollution and of the environmental conditions .
	manualset3
95128	7	400651	13	NULL	NULL	0	NULL	 urban wastes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mussels from station C , located in the channel from the lagoon to the Mediterranean and submitted to pollutants ( urban wastes from Bizerta and hydrocarbons from the maritime traffic ) , acetylcholinesterase activities were lower than in those from station J. In conclusion , the variations in acetylcholinesterase activity observed between stations in both species may be the result of pollution and of the environmental conditions .
	manualset3
95129	8	400651	13	NULL	NULL	0	NULL	Bizerta 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mussels from station C , located in the channel from the lagoon to the Mediterranean and submitted to pollutants ( urban wastes from Bizerta and hydrocarbons from the maritime traffic ) , acetylcholinesterase activities were lower than in those from station J. In conclusion , the variations in acetylcholinesterase activity observed between stations in both species may be the result of pollution and of the environmental conditions .
	manualset3
95130	9	400651	13	NULL	NULL	0	NULL	hydrocarbons	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mussels from station C , located in the channel from the lagoon to the Mediterranean and submitted to pollutants ( urban wastes from Bizerta and hydrocarbons from the maritime traffic ) , acetylcholinesterase activities were lower than in those from station J. In conclusion , the variations in acetylcholinesterase activity observed between stations in both species may be the result of pollution and of the environmental conditions .
	manualset3
95132	10	400651	13	NULL	NULL	0	NULL	maritime traffic	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mussels from station C , located in the channel from the lagoon to the Mediterranean and submitted to pollutants ( urban wastes from Bizerta and hydrocarbons from the maritime traffic ) , acetylcholinesterase activities were lower than in those from station J. In conclusion , the variations in acetylcholinesterase activity observed between stations in both species may be the result of pollution and of the environmental conditions .
	manualset3
95133	11	400651	13	NULL	NULL	0	NULL	acetylcholinesterase activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mussels from station C , located in the channel from the lagoon to the Mediterranean and submitted to pollutants ( urban wastes from Bizerta and hydrocarbons from the maritime traffic ) , acetylcholinesterase activities were lower than in those from station J. In conclusion , the variations in acetylcholinesterase activity observed between stations in both species may be the result of pollution and of the environmental conditions .
	manualset3
95134	12	400651	13	NULL	NULL	0	NULL	station J	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mussels from station C , located in the channel from the lagoon to the Mediterranean and submitted to pollutants ( urban wastes from Bizerta and hydrocarbons from the maritime traffic ) , acetylcholinesterase activities were lower than in those from station J. In conclusion , the variations in acetylcholinesterase activity observed between stations in both species may be the result of pollution and of the environmental conditions .
	manualset3
95135	13	400651	13	NULL	NULL	0	NULL	conclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mussels from station C , located in the channel from the lagoon to the Mediterranean and submitted to pollutants ( urban wastes from Bizerta and hydrocarbons from the maritime traffic ) , acetylcholinesterase activities were lower than in those from station J. In conclusion , the variations in acetylcholinesterase activity observed between stations in both species may be the result of pollution and of the environmental conditions .
	manualset3
95136	14	400651	13	NULL	NULL	0	NULL	variations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mussels from station C , located in the channel from the lagoon to the Mediterranean and submitted to pollutants ( urban wastes from Bizerta and hydrocarbons from the maritime traffic ) , acetylcholinesterase activities were lower than in those from station J. In conclusion , the variations in acetylcholinesterase activity observed between stations in both species may be the result of pollution and of the environmental conditions .
	manualset3
95137	15	400651	13	NULL	NULL	0	NULL	acetylcholinesterase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mussels from station C , located in the channel from the lagoon to the Mediterranean and submitted to pollutants ( urban wastes from Bizerta and hydrocarbons from the maritime traffic ) , acetylcholinesterase activities were lower than in those from station J. In conclusion , the variations in acetylcholinesterase activity observed between stations in both species may be the result of pollution and of the environmental conditions .
	manualset3
95138	16	400651	13	NULL	NULL	0	NULL	stations	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mussels from station C , located in the channel from the lagoon to the Mediterranean and submitted to pollutants ( urban wastes from Bizerta and hydrocarbons from the maritime traffic ) , acetylcholinesterase activities were lower than in those from station J. In conclusion , the variations in acetylcholinesterase activity observed between stations in both species may be the result of pollution and of the environmental conditions .
	manualset3
95139	17	400651	13	NULL	NULL	0	NULL	species 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mussels from station C , located in the channel from the lagoon to the Mediterranean and submitted to pollutants ( urban wastes from Bizerta and hydrocarbons from the maritime traffic ) , acetylcholinesterase activities were lower than in those from station J. In conclusion , the variations in acetylcholinesterase activity observed between stations in both species may be the result of pollution and of the environmental conditions .
	manualset3
95140	18	400651	13	NULL	NULL	0	NULL	result	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mussels from station C , located in the channel from the lagoon to the Mediterranean and submitted to pollutants ( urban wastes from Bizerta and hydrocarbons from the maritime traffic ) , acetylcholinesterase activities were lower than in those from station J. In conclusion , the variations in acetylcholinesterase activity observed between stations in both species may be the result of pollution and of the environmental conditions .
	manualset3
95141	19	400651	13	NULL	NULL	0	NULL	pollution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mussels from station C , located in the channel from the lagoon to the Mediterranean and submitted to pollutants ( urban wastes from Bizerta and hydrocarbons from the maritime traffic ) , acetylcholinesterase activities were lower than in those from station J. In conclusion , the variations in acetylcholinesterase activity observed between stations in both species may be the result of pollution and of the environmental conditions .
	manualset3
95142	20	400651	13	NULL	NULL	0	NULL	environmental conditions	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mussels from station C , located in the channel from the lagoon to the Mediterranean and submitted to pollutants ( urban wastes from Bizerta and hydrocarbons from the maritime traffic ) , acetylcholinesterase activities were lower than in those from station J. In conclusion , the variations in acetylcholinesterase activity observed between stations in both species may be the result of pollution and of the environmental conditions .
	manualset3
95143	1	400652	13	NULL	NULL	0	NULL	 mutants ' brains	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mutants ' brains , entry of T4 was not affected , but uptake of T3 was diminished .
	manualset3
95144	2	400652	13	NULL	NULL	0	NULL	entry 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mutants ' brains , entry of T4 was not affected , but uptake of T3 was diminished .
	manualset3
95145	3	400652	13	NULL	NULL	0	NULL	 T4	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mutants ' brains , entry of T4 was not affected , but uptake of T3 was diminished .
	manualset3
95146	4	400652	13	NULL	NULL	0	NULL	uptake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mutants ' brains , entry of T4 was not affected , but uptake of T3 was diminished .
	manualset3
95147	5	400652	13	NULL	NULL	0	NULL	T3 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the mutants ' brains , entry of T4 was not affected , but uptake of T3 was diminished .
	manualset3
95148	1	400653	13	NULL	NULL	NULL	NULL	nine years	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the nine years since the Global Advisory Group of the Expanded Programme on Immunisation ( WHO ) set 1997 as the target for integrating hepatitis B vaccination into national immunisation programs worldwide , 129 countries have included hepatitis B vaccine as part of their routine infant or adolescent immunisation programs ( June 2001 ) .
	manualset3
95149	2	400653	13	NULL	NULL	0	NULL	 Global Advisory Group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the nine years since the Global Advisory Group of the Expanded Programme on Immunisation ( WHO ) set 1997 as the target for integrating hepatitis B vaccination into national immunisation programs worldwide , 129 countries have included hepatitis B vaccine as part of their routine infant or adolescent immunisation programs ( June 2001 ) .
	manualset3
95150	3	400653	13	NULL	NULL	NULL	NULL	Expanded Programme on Immunisation ( WHO ) 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the nine years since the Global Advisory Group of the Expanded Programme on Immunisation ( WHO ) set 1997 as the target for integrating hepatitis B vaccination into national immunisation programs worldwide , 129 countries have included hepatitis B vaccine as part of their routine infant or adolescent immunisation programs ( June 2001 ) .
	manualset3
95151	4	400653	13	NULL	NULL	0	NULL	1997	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In the nine years since the Global Advisory Group of the Expanded Programme on Immunisation ( WHO ) set 1997 as the target for integrating hepatitis B vaccination into national immunisation programs worldwide , 129 countries have included hepatitis B vaccine as part of their routine infant or adolescent immunisation programs ( June 2001 ) .
	manualset3
95152	5	400653	13	NULL	NULL	0	NULL	target 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the nine years since the Global Advisory Group of the Expanded Programme on Immunisation ( WHO ) set 1997 as the target for integrating hepatitis B vaccination into national immunisation programs worldwide , 129 countries have included hepatitis B vaccine as part of their routine infant or adolescent immunisation programs ( June 2001 ) .
	manualset3
95153	6	400653	13	NULL	NULL	0	NULL	 hepatitis B vaccination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the nine years since the Global Advisory Group of the Expanded Programme on Immunisation ( WHO ) set 1997 as the target for integrating hepatitis B vaccination into national immunisation programs worldwide , 129 countries have included hepatitis B vaccine as part of their routine infant or adolescent immunisation programs ( June 2001 ) .
	manualset3
95154	7	400653	13	NULL	NULL	0	NULL	national immunisation programs worldwide 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the nine years since the Global Advisory Group of the Expanded Programme on Immunisation ( WHO ) set 1997 as the target for integrating hepatitis B vaccination into national immunisation programs worldwide , 129 countries have included hepatitis B vaccine as part of their routine infant or adolescent immunisation programs ( June 2001 ) .
	manualset3
95155	8	400653	13	NULL	NULL	0	NULL	129 countries 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the nine years since the Global Advisory Group of the Expanded Programme on Immunisation ( WHO ) set 1997 as the target for integrating hepatitis B vaccination into national immunisation programs worldwide , 129 countries have included hepatitis B vaccine as part of their routine infant or adolescent immunisation programs ( June 2001 ) .
	manualset3
95156	9	400653	13	NULL	NULL	0	NULL	hepatitis B vaccine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the nine years since the Global Advisory Group of the Expanded Programme on Immunisation ( WHO ) set 1997 as the target for integrating hepatitis B vaccination into national immunisation programs worldwide , 129 countries have included hepatitis B vaccine as part of their routine infant or adolescent immunisation programs ( June 2001 ) .
	manualset3
95157	10	400653	13	NULL	NULL	0	NULL	routine infant immunisation programs	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the nine years since the Global Advisory Group of the Expanded Programme on Immunisation ( WHO ) set 1997 as the target for integrating hepatitis B vaccination into national immunisation programs worldwide , 129 countries have included hepatitis B vaccine as part of their routine infant or adolescent immunisation programs ( June 2001 ) .
	manualset3
95158	11	400653	13	NULL	NULL	0	NULL	adolescent immunisation programs 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the nine years since the Global Advisory Group of the Expanded Programme on Immunisation ( WHO ) set 1997 as the target for integrating hepatitis B vaccination into national immunisation programs worldwide , 129 countries have included hepatitis B vaccine as part of their routine infant or adolescent immunisation programs ( June 2001 ) .
	manualset3
95159	12	400653	13	NULL	NULL	0	NULL	June 2001 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In the nine years since the Global Advisory Group of the Expanded Programme on Immunisation ( WHO ) set 1997 as the target for integrating hepatitis B vaccination into national immunisation programs worldwide , 129 countries have included hepatitis B vaccine as part of their routine infant or adolescent immunisation programs ( June 2001 ) .
	manualset3
95160	1	400654	13	NULL	NULL	0	NULL	1 month	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	1 month after the resection both glycogen content and rat liver cell morphology were seen almost close to the normal .
	manualset3
95161	2	400654	13	NULL	NULL	NULL	NULL	glycogen content	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	1 month after the resection both glycogen content and rat liver cell morphology were seen almost close to the normal .
	manualset3
95162	3	400654	13	NULL	NULL	0	NULL	rat liver cell morphology	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	1 month after the resection both glycogen content and rat liver cell morphology were seen almost close to the normal .
	manualset3
98582	4	400654	13	NULL	NULL	0	NULL	resection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	1 month after the resection both glycogen content and rat liver cell morphology were seen almost close to the normal .
	manualset3
95163	1	400655	13	NULL	NULL	0	NULL	non-responder patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In the non-responder patient the internalization of EGF receptor ligand was decreased , whereas it was increased in the fibroblasts derived from the responder patient after PHT therapy .
	manualset3
95164	2	400655	13	NULL	NULL	NULL	NULL	internalization of EGF receptor ligand	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the non-responder patient the internalization of EGF receptor ligand was decreased , whereas it was increased in the fibroblasts derived from the responder patient after PHT therapy .
	manualset3
95165	3	400655	13	NULL	NULL	0	NULL	fibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the non-responder patient the internalization of EGF receptor ligand was decreased , whereas it was increased in the fibroblasts derived from the responder patient after PHT therapy .
	manualset3
95166	4	400655	13	NULL	NULL	0	NULL	responder patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In the non-responder patient the internalization of EGF receptor ligand was decreased , whereas it was increased in the fibroblasts derived from the responder patient after PHT therapy .
	manualset3
95167	5	400655	13	NULL	NULL	0	NULL	 PHT therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the non-responder patient the internalization of EGF receptor ligand was decreased , whereas it was increased in the fibroblasts derived from the responder patient after PHT therapy .
	manualset3
95168	1	400656	13	NULL	NULL	0	NULL	normal adrenal cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the normal adrenal cell , epinephrine does not activate the rise of either cGMP or cAMP concentrations .
	manualset3
95169	2	400656	13	NULL	NULL	0	NULL	epinephrine	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the normal adrenal cell , epinephrine does not activate the rise of either cGMP or cAMP concentrations .
	manualset3
95170	3	400656	13	NULL	NULL	0	NULL	 rise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the normal adrenal cell , epinephrine does not activate the rise of either cGMP or cAMP concentrations .
	manualset3
95171	4	400656	13	NULL	NULL	0	NULL	cGMP concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the normal adrenal cell , epinephrine does not activate the rise of either cGMP or cAMP concentrations .
	manualset3
95172	5	400656	13	NULL	NULL	0	NULL	 cAMP concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the normal adrenal cell , epinephrine does not activate the rise of either cGMP or cAMP concentrations .
	manualset3
95173	1	400657	13	NULL	NULL	0	NULL	old strategy	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In the old strategy , endoscopy was performed on patients with dyspepsia , in the hope of detecting a treatable peptic ulcer .
	manualset3
95174	2	400657	13	NULL	NULL	0	NULL	endoscopy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the old strategy , endoscopy was performed on patients with dyspepsia , in the hope of detecting a treatable peptic ulcer .
	manualset3
95175	3	400657	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the old strategy , endoscopy was performed on patients with dyspepsia , in the hope of detecting a treatable peptic ulcer .
	manualset3
95176	4	400657	13	NULL	NULL	0	NULL	dyspepsia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the old strategy , endoscopy was performed on patients with dyspepsia , in the hope of detecting a treatable peptic ulcer .
	manualset3
95177	5	400657	13	NULL	NULL	0	NULL	hope	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the old strategy , endoscopy was performed on patients with dyspepsia , in the hope of detecting a treatable peptic ulcer .
	manualset3
95178	6	400657	13	NULL	NULL	0	NULL	peptic ulcer	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the old strategy , endoscopy was performed on patients with dyspepsia , in the hope of detecting a treatable peptic ulcer .
	manualset3
95179	1	400658	13	NULL	NULL	0	NULL	olfactory pathway	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the olfactory pathway of the moth Manduca sexta , we find that different odorants evoke gamma-band oscillations in the AL and the mushroom body ( a higher-order network that receives input from the AL ) , but oscillations within or between these two processing stages are not temporally coherent .
	manualset3
95180	2	400658	13	NULL	NULL	0	NULL	 moth Manduca sexta	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the olfactory pathway of the moth Manduca sexta , we find that different odorants evoke gamma-band oscillations in the AL and the mushroom body ( a higher-order network that receives input from the AL ) , but oscillations within or between these two processing stages are not temporally coherent .
	manualset3
95181	3	400658	13	NULL	NULL	0	NULL	 odorants 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the olfactory pathway of the moth Manduca sexta , we find that different odorants evoke gamma-band oscillations in the AL and the mushroom body ( a higher-order network that receives input from the AL ) , but oscillations within or between these two processing stages are not temporally coherent .
	manualset3
95182	4	400658	13	NULL	NULL	0	NULL	gamma-band oscillations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the olfactory pathway of the moth Manduca sexta , we find that different odorants evoke gamma-band oscillations in the AL and the mushroom body ( a higher-order network that receives input from the AL ) , but oscillations within or between these two processing stages are not temporally coherent .
	manualset3
95183	5	400658	13	NULL	NULL	0	NULL	AL	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the olfactory pathway of the moth Manduca sexta , we find that different odorants evoke gamma-band oscillations in the AL and the mushroom body ( a higher-order network that receives input from the AL ) , but oscillations within or between these two processing stages are not temporally coherent .
	manualset3
95184	6	400658	13	NULL	NULL	0	NULL	mushroom body	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the olfactory pathway of the moth Manduca sexta , we find that different odorants evoke gamma-band oscillations in the AL and the mushroom body ( a higher-order network that receives input from the AL ) , but oscillations within or between these two processing stages are not temporally coherent .
	manualset3
95185	7	400658	13	NULL	NULL	0	NULL	higher-order network	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the olfactory pathway of the moth Manduca sexta , we find that different odorants evoke gamma-band oscillations in the AL and the mushroom body ( a higher-order network that receives input from the AL ) , but oscillations within or between these two processing stages are not temporally coherent .
	manualset3
95186	8	400658	13	NULL	NULL	0	NULL	input 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the olfactory pathway of the moth Manduca sexta , we find that different odorants evoke gamma-band oscillations in the AL and the mushroom body ( a higher-order network that receives input from the AL ) , but oscillations within or between these two processing stages are not temporally coherent .
	manualset3
95187	9	400658	13	NULL	NULL	0	NULL	AL	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the olfactory pathway of the moth Manduca sexta , we find that different odorants evoke gamma-band oscillations in the AL and the mushroom body ( a higher-order network that receives input from the AL ) , but oscillations within or between these two processing stages are not temporally coherent .
	manualset3
95188	10	400658	13	NULL	NULL	0	NULL	oscillations 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the olfactory pathway of the moth Manduca sexta , we find that different odorants evoke gamma-band oscillations in the AL and the mushroom body ( a higher-order network that receives input from the AL ) , but oscillations within or between these two processing stages are not temporally coherent .
	manualset3
95189	11	400658	13	NULL	NULL	0	NULL	two processing stages	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the olfactory pathway of the moth Manduca sexta , we find that different odorants evoke gamma-band oscillations in the AL and the mushroom body ( a higher-order network that receives input from the AL ) , but oscillations within or between these two processing stages are not temporally coherent .
	manualset3
95191	1	400659	13	NULL	NULL	0	NULL	orbital layer	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the orbital layer of all three muscles examined , the large numbers of fibers positive for fast MHC in the middle of the muscle dramatically decreased at the tendon end , with a concomitant increase in expression of slow myosin .
	manualset3
95192	2	400659	13	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the orbital layer of all three muscles examined , the large numbers of fibers positive for fast MHC in the middle of the muscle dramatically decreased at the tendon end , with a concomitant increase in expression of slow myosin .
	manualset3
95193	3	400659	13	NULL	NULL	0	NULL	muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the orbital layer of all three muscles examined , the large numbers of fibers positive for fast MHC in the middle of the muscle dramatically decreased at the tendon end , with a concomitant increase in expression of slow myosin .
	manualset3
95194	4	400659	13	NULL	NULL	0	NULL	large numbers of fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the orbital layer of all three muscles examined , the large numbers of fibers positive for fast MHC in the middle of the muscle dramatically decreased at the tendon end , with a concomitant increase in expression of slow myosin .
	manualset3
95198	5	400659	13	NULL	NULL	0	NULL	 MHC 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the orbital layer of all three muscles examined , the large numbers of fibers positive for fast MHC in the middle of the muscle dramatically decreased at the tendon end , with a concomitant increase in expression of slow myosin .
	manualset3
95199	6	400659	13	NULL	NULL	0	NULL	middle of the muscle 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the orbital layer of all three muscles examined , the large numbers of fibers positive for fast MHC in the middle of the muscle dramatically decreased at the tendon end , with a concomitant increase in expression of slow myosin .
	manualset3
95200	7	400659	13	NULL	NULL	0	NULL	 tendon end	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the orbital layer of all three muscles examined , the large numbers of fibers positive for fast MHC in the middle of the muscle dramatically decreased at the tendon end , with a concomitant increase in expression of slow myosin .
	manualset3
95201	8	400659	13	NULL	NULL	0	NULL	increase in expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the orbital layer of all three muscles examined , the large numbers of fibers positive for fast MHC in the middle of the muscle dramatically decreased at the tendon end , with a concomitant increase in expression of slow myosin .
	manualset3
95202	9	400659	13	NULL	NULL	0	NULL	 myosin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the orbital layer of all three muscles examined , the large numbers of fibers positive for fast MHC in the middle of the muscle dramatically decreased at the tendon end , with a concomitant increase in expression of slow myosin .
	manualset3
95203	1	400660	13	NULL	NULL	0	NULL	16	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the other 16 patients laser treatment alone ( 8 ) or in conjunction with electroresection ( 8 ) eradicated the tumor successfully .
	manualset3
95204	2	400660	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the other 16 patients laser treatment alone ( 8 ) or in conjunction with electroresection ( 8 ) eradicated the tumor successfully .
	manualset3
95205	3	400660	13	NULL	NULL	0	NULL	 laser treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the other 16 patients laser treatment alone ( 8 ) or in conjunction with electroresection ( 8 ) eradicated the tumor successfully .
	manualset3
95208	4	400660	13	NULL	NULL	0	NULL	8	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the other 16 patients laser treatment alone ( 8 ) or in conjunction with electroresection ( 8 ) eradicated the tumor successfully .
	manualset3
95210	5	400660	13	NULL	NULL	0	NULL	conjunction with electroresection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the other 16 patients laser treatment alone ( 8 ) or in conjunction with electroresection ( 8 ) eradicated the tumor successfully .
	manualset3
95211	6	400660	13	NULL	NULL	0	NULL	 8 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the other 16 patients laser treatment alone ( 8 ) or in conjunction with electroresection ( 8 ) eradicated the tumor successfully .
	manualset3
95213	7	400660	13	NULL	NULL	0	NULL	tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the other 16 patients laser treatment alone ( 8 ) or in conjunction with electroresection ( 8 ) eradicated the tumor successfully .
	manualset3
95258	1	400661	13	NULL	NULL	0	NULL	 conformation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the other conformation , the nicotinamide is too far from the enzyme-substrate adduct for efficient hydride transfer .
	manualset3
95262	2	400661	13	NULL	NULL	0	NULL	nicotinamide	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the other conformation , the nicotinamide is too far from the enzyme-substrate adduct for efficient hydride transfer .
	manualset3
95268	3	400661	13	NULL	NULL	0	NULL	enzyme-substrate adduct	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the other conformation , the nicotinamide is too far from the enzyme-substrate adduct for efficient hydride transfer .
	manualset3
95270	4	400661	13	NULL	NULL	0	NULL	hydride transfer	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the other conformation , the nicotinamide is too far from the enzyme-substrate adduct for efficient hydride transfer .
	manualset3
95274	1	400662	13	NULL	NULL	0	NULL	four	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the other four cases , including three cases of diabetic ketoacidosis , no identifiable triggering events were present .
	manualset3
95275	2	400662	13	NULL	NULL	NULL	NULL	cases	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the other four cases , including three cases of diabetic ketoacidosis , no identifiable triggering events were present .
	manualset3
95277	3	400662	13	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the other four cases , including three cases of diabetic ketoacidosis , no identifiable triggering events were present .
	manualset3
95279	4	400662	13	NULL	NULL	NULL	NULL	cases 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the other four cases , including three cases of diabetic ketoacidosis , no identifiable triggering events were present .
	manualset3
95280	5	400662	13	NULL	NULL	0	NULL	diabetic ketoacidosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the other four cases , including three cases of diabetic ketoacidosis , no identifiable triggering events were present .
	manualset3
95282	6	400662	13	NULL	NULL	0	NULL	triggering events	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the other four cases , including three cases of diabetic ketoacidosis , no identifiable triggering events were present .
	manualset3
95311	1	400663	13	NULL	NULL	0	NULL	2	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Apropos of 2 cases of intestinal invagination in infants caused by Meckel 's diverticulum and of a case of invagination caused by an enterocystoma of Bauhin 's valve ) .
	manualset3
95312	2	400663	13	NULL	NULL	0	NULL	cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Apropos of 2 cases of intestinal invagination in infants caused by Meckel 's diverticulum and of a case of invagination caused by an enterocystoma of Bauhin 's valve ) .
	manualset3
95313	3	400663	13	NULL	NULL	0	NULL	intestinal invagination	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Apropos of 2 cases of intestinal invagination in infants caused by Meckel 's diverticulum and of a case of invagination caused by an enterocystoma of Bauhin 's valve ) .
	manualset3
95314	4	400663	13	NULL	NULL	0	NULL	 infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Apropos of 2 cases of intestinal invagination in infants caused by Meckel 's diverticulum and of a case of invagination caused by an enterocystoma of Bauhin 's valve ) .
	manualset3
95315	5	400663	13	NULL	NULL	0	NULL	Meckel 's diverticulum	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Apropos of 2 cases of intestinal invagination in infants caused by Meckel 's diverticulum and of a case of invagination caused by an enterocystoma of Bauhin 's valve ) .
	manualset3
95316	6	400663	13	NULL	NULL	0	NULL	case 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( Apropos of 2 cases of intestinal invagination in infants caused by Meckel 's diverticulum and of a case of invagination caused by an enterocystoma of Bauhin 's valve ) .
	manualset3
95317	7	400663	13	NULL	NULL	0	NULL	invagination 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Apropos of 2 cases of intestinal invagination in infants caused by Meckel 's diverticulum and of a case of invagination caused by an enterocystoma of Bauhin 's valve ) .
	manualset3
95318	8	400663	13	NULL	NULL	0	NULL	 enterocystoma of Bauhin 's valve	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Apropos of 2 cases of intestinal invagination in infants caused by Meckel 's diverticulum and of a case of invagination caused by an enterocystoma of Bauhin 's valve ) .
	manualset3
95319	1	400664	13	NULL	NULL	0	NULL	paraventricular nucleus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the paraventricular nucleus from morphine-withdrawn rats , the number of neurons expressing CRF was increased .
	manualset3
95320	2	400664	13	NULL	NULL	0	NULL	 morphine-withdrawn rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the paraventricular nucleus from morphine-withdrawn rats , the number of neurons expressing CRF was increased .
	manualset3
95321	3	400664	13	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the paraventricular nucleus from morphine-withdrawn rats , the number of neurons expressing CRF was increased .
	manualset3
95322	4	400664	13	NULL	NULL	NULL	NULL	neurons	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the paraventricular nucleus from morphine-withdrawn rats , the number of neurons expressing CRF was increased .
	manualset3
95323	5	400664	13	NULL	NULL	0	NULL	CRF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the paraventricular nucleus from morphine-withdrawn rats , the number of neurons expressing CRF was increased .
	manualset3
95324	1	400665	13	NULL	NULL	0	NULL	particles	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the particles of the DI engine , the organic carbon contributed 14-26 % to the total carbon emissions , the advanced engine technology , and the oxidation catalyst , thus reducing the OC/EC ratio of particles considerably .
	manualset3
95325	2	400665	13	NULL	NULL	0	NULL	DI engine	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In the particles of the DI engine , the organic carbon contributed 14-26 % to the total carbon emissions , the advanced engine technology , and the oxidation catalyst , thus reducing the OC/EC ratio of particles considerably .
	manualset3
95326	3	400665	13	NULL	NULL	0	NULL	 organic carbon	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the particles of the DI engine , the organic carbon contributed 14-26 % to the total carbon emissions , the advanced engine technology , and the oxidation catalyst , thus reducing the OC/EC ratio of particles considerably .
	manualset3
95327	4	400665	13	NULL	NULL	0	NULL	 14-26 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the particles of the DI engine , the organic carbon contributed 14-26 % to the total carbon emissions , the advanced engine technology , and the oxidation catalyst , thus reducing the OC/EC ratio of particles considerably .
	manualset3
95328	5	400665	13	NULL	NULL	0	NULL	total carbon emissions	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the particles of the DI engine , the organic carbon contributed 14-26 % to the total carbon emissions , the advanced engine technology , and the oxidation catalyst , thus reducing the OC/EC ratio of particles considerably .
	manualset3
95329	6	400665	13	NULL	NULL	0	NULL	engine technology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In the particles of the DI engine , the organic carbon contributed 14-26 % to the total carbon emissions , the advanced engine technology , and the oxidation catalyst , thus reducing the OC/EC ratio of particles considerably .
	manualset3
95330	7	400665	13	NULL	NULL	0	NULL	oxidation catalyst	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the particles of the DI engine , the organic carbon contributed 14-26 % to the total carbon emissions , the advanced engine technology , and the oxidation catalyst , thus reducing the OC/EC ratio of particles considerably .
	manualset3
95331	8	400665	13	NULL	NULL	0	NULL	OC/EC ratio	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the particles of the DI engine , the organic carbon contributed 14-26 % to the total carbon emissions , the advanced engine technology , and the oxidation catalyst , thus reducing the OC/EC ratio of particles considerably .
	manualset3
95332	9	400665	13	NULL	NULL	0	NULL	particles	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the particles of the DI engine , the organic carbon contributed 14-26 % to the total carbon emissions , the advanced engine technology , and the oxidation catalyst , thus reducing the OC/EC ratio of particles considerably .
	manualset3
95333	1	400666	13	NULL	NULL	0	NULL	passengers group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the passengers group , holding the driver or others responsible led , mediated by increased self-blame , feelings of guilt , and family distress , to lower psychological well-being ( PWB ) .
	manualset3
95334	2	400666	13	NULL	NULL	0	NULL	driver	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In the passengers group , holding the driver or others responsible led , mediated by increased self-blame , feelings of guilt , and family distress , to lower psychological well-being ( PWB ) .
	manualset3
95335	3	400666	13	NULL	NULL	0	NULL	others	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the passengers group , holding the driver or others responsible led , mediated by increased self-blame , feelings of guilt , and family distress , to lower psychological well-being ( PWB ) .
	manualset3
95336	4	400666	13	NULL	NULL	0	NULL	feelings of guilt	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the passengers group , holding the driver or others responsible led , mediated by increased self-blame , feelings of guilt , and family distress , to lower psychological well-being ( PWB ) .
	manualset3
95337	5	400666	13	NULL	NULL	0	NULL	family	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the passengers group , holding the driver or others responsible led , mediated by increased self-blame , feelings of guilt , and family distress , to lower psychological well-being ( PWB ) .
	manualset3
95338	6	400666	13	NULL	NULL	0	NULL	distress	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the passengers group , holding the driver or others responsible led , mediated by increased self-blame , feelings of guilt , and family distress , to lower psychological well-being ( PWB ) .
	manualset3
95339	7	400666	13	NULL	NULL	0	NULL	psychological well-being ( PWB )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the passengers group , holding the driver or others responsible led , mediated by increased self-blame , feelings of guilt , and family distress , to lower psychological well-being ( PWB ) .
	manualset3
98583	8	400666	13	NULL	NULL	0	NULL	self-blame	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the passengers group , holding the driver or others responsible led , mediated by increased self-blame , feelings of guilt , and family distress , to lower psychological well-being ( PWB ) .
	manualset3
95340	1	400667	13	NULL	NULL	0	NULL	past decades	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past decades , many pharmacological reagents have been identified that regulate this pathway at the level of the receptor .
	manualset3
95341	2	400667	13	NULL	NULL	0	NULL	pharmacological reagents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past decades , many pharmacological reagents have been identified that regulate this pathway at the level of the receptor .
	manualset3
95342	3	400667	13	NULL	NULL	0	NULL	pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past decades , many pharmacological reagents have been identified that regulate this pathway at the level of the receptor .
	manualset3
95343	4	400667	13	NULL	NULL	0	NULL	level of the receptor 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past decades , many pharmacological reagents have been identified that regulate this pathway at the level of the receptor .
	manualset3
95344	1	400668	13	NULL	NULL	0	NULL	past five years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past five years in vitro models have been developed to characterize interaction of HCV glycoproteins with host cell entry factors and detect antibodies interfering with HCV entry and infection .
	manualset3
95346	2	400668	13	NULL	NULL	0	NULL	in vitro models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past five years in vitro models have been developed to characterize interaction of HCV glycoproteins with host cell entry factors and detect antibodies interfering with HCV entry and infection .
	manualset3
95347	3	400668	13	NULL	NULL	0	NULL	 interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past five years in vitro models have been developed to characterize interaction of HCV glycoproteins with host cell entry factors and detect antibodies interfering with HCV entry and infection .
	manualset3
95348	4	400668	13	NULL	NULL	0	NULL	HCV glycoproteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past five years in vitro models have been developed to characterize interaction of HCV glycoproteins with host cell entry factors and detect antibodies interfering with HCV entry and infection .
	manualset3
95352	5	400668	13	NULL	NULL	NULL	NULL	host cell entry factors 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the past five years in vitro models have been developed to characterize interaction of HCV glycoproteins with host cell entry factors and detect antibodies interfering with HCV entry and infection .
	manualset3
95353	6	400668	13	NULL	NULL	0	NULL	antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past five years in vitro models have been developed to characterize interaction of HCV glycoproteins with host cell entry factors and detect antibodies interfering with HCV entry and infection .
	manualset3
95354	7	400668	13	NULL	NULL	0	NULL	HCV entry 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past five years in vitro models have been developed to characterize interaction of HCV glycoproteins with host cell entry factors and detect antibodies interfering with HCV entry and infection .
	manualset3
95356	8	400668	13	NULL	NULL	0	NULL	infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past five years in vitro models have been developed to characterize interaction of HCV glycoproteins with host cell entry factors and detect antibodies interfering with HCV entry and infection .
	manualset3
95359	1	400669	13	NULL	NULL	0	NULL	past year 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past year , critical information was derived from animal models that mimic human cardiac hypertrophy and failure .
	manualset3
95361	2	400669	13	NULL	NULL	0	NULL	critical information	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past year , critical information was derived from animal models that mimic human cardiac hypertrophy and failure .
	manualset3
95363	3	400669	13	NULL	NULL	0	NULL	animal models	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past year , critical information was derived from animal models that mimic human cardiac hypertrophy and failure .
	manualset3
95364	4	400669	13	NULL	NULL	0	NULL	human cardiac hypertrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past year , critical information was derived from animal models that mimic human cardiac hypertrophy and failure .
	manualset3
95365	5	400669	13	NULL	NULL	0	NULL	human cardiac failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past year , critical information was derived from animal models that mimic human cardiac hypertrophy and failure .
	manualset3
95366	1	400670	13	NULL	NULL	0	NULL	past	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past , short-term internal treatment with griseofulvin and ketoconazole resulted in fast clearing of skin symptoms .
	manualset3
95367	2	400670	13	NULL	NULL	0	NULL	short-term internal treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past , short-term internal treatment with griseofulvin and ketoconazole resulted in fast clearing of skin symptoms .
	manualset3
95368	3	400670	13	NULL	NULL	0	NULL	griseofulvin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past , short-term internal treatment with griseofulvin and ketoconazole resulted in fast clearing of skin symptoms .
	manualset3
95369	4	400670	13	NULL	NULL	0	NULL	ketoconazole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past , short-term internal treatment with griseofulvin and ketoconazole resulted in fast clearing of skin symptoms .
	manualset3
95370	5	400670	13	NULL	NULL	0	NULL	skin symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past , short-term internal treatment with griseofulvin and ketoconazole resulted in fast clearing of skin symptoms .
	manualset3
95371	1	400671	13	NULL	NULL	0	NULL	period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the period between 1.1.1974 and 31.12.1978 phage typing of 2058 strains of S. typhi and 1672 strains of S. paratyphi-B was carried out .
	manualset3
95372	2	400671	13	NULL	NULL	0	NULL	1.1.1974	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In the period between 1.1.1974 and 31.12.1978 phage typing of 2058 strains of S. typhi and 1672 strains of S. paratyphi-B was carried out .
	manualset3
95373	3	400671	13	NULL	NULL	0	NULL	31.12.1978	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In the period between 1.1.1974 and 31.12.1978 phage typing of 2058 strains of S. typhi and 1672 strains of S. paratyphi-B was carried out .
	manualset3
95374	4	400671	13	NULL	NULL	0	NULL	phage typing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the period between 1.1.1974 and 31.12.1978 phage typing of 2058 strains of S. typhi and 1672 strains of S. paratyphi-B was carried out .
	manualset3
95375	5	400671	13	NULL	NULL	NULL	NULL	2058 strains 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the period between 1.1.1974 and 31.12.1978 phage typing of 2058 strains of S. typhi and 1672 strains of S. paratyphi-B was carried out .
	manualset3
95376	6	400671	13	NULL	NULL	0	NULL	S. typhi	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the period between 1.1.1974 and 31.12.1978 phage typing of 2058 strains of S. typhi and 1672 strains of S. paratyphi-B was carried out .
	manualset3
95377	7	400671	13	NULL	NULL	NULL	NULL	1672 strains	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the period between 1.1.1974 and 31.12.1978 phage typing of 2058 strains of S. typhi and 1672 strains of S. paratyphi-B was carried out .
	manualset3
95378	8	400671	13	NULL	NULL	0	NULL	S. paratyphi-B	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the period between 1.1.1974 and 31.12.1978 phage typing of 2058 strains of S. typhi and 1672 strains of S. paratyphi-B was carried out .
	manualset3
95379	1	400672	13	NULL	NULL	0	NULL	 polypeptide fragment	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	In the polypeptide fragment , this epitope forms a stable , amphipathic , alpha helix under organic and membrane-mimetic conditions , but has only a partially helical conformation in aqueous solution .
	manualset3
95380	2	400672	13	NULL	NULL	0	NULL	epitope 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	In the polypeptide fragment , this epitope forms a stable , amphipathic , alpha helix under organic and membrane-mimetic conditions , but has only a partially helical conformation in aqueous solution .
	manualset3
95381	3	400672	13	NULL	NULL	0	NULL	alpha helix 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	In the polypeptide fragment , this epitope forms a stable , amphipathic , alpha helix under organic and membrane-mimetic conditions , but has only a partially helical conformation in aqueous solution .
	manualset3
95382	4	400672	13	NULL	NULL	NULL	NULL	organic conditions	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the polypeptide fragment , this epitope forms a stable , amphipathic , alpha helix under organic and membrane-mimetic conditions , but has only a partially helical conformation in aqueous solution .
	manualset3
95383	5	400672	13	NULL	NULL	NULL	NULL	membrane-mimetic conditions	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the polypeptide fragment , this epitope forms a stable , amphipathic , alpha helix under organic and membrane-mimetic conditions , but has only a partially helical conformation in aqueous solution .
	manualset3
95384	6	400672	13	NULL	NULL	0	NULL	helical conformation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the polypeptide fragment , this epitope forms a stable , amphipathic , alpha helix under organic and membrane-mimetic conditions , but has only a partially helical conformation in aqueous solution .
	manualset3
95385	7	400672	13	NULL	NULL	0	NULL	aqueous solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the polypeptide fragment , this epitope forms a stable , amphipathic , alpha helix under organic and membrane-mimetic conditions , but has only a partially helical conformation in aqueous solution .
	manualset3
95386	1	400673	13	NULL	NULL	0	NULL	prefrontal cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the prefrontal cortex , handling reduced thiol content and appears to imbalance the antioxidant enzymes system , which is counteracted by a palatable diet .
	manualset3
95387	2	400673	13	NULL	NULL	NULL	NULL	handling	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the prefrontal cortex , handling reduced thiol content and appears to imbalance the antioxidant enzymes system , which is counteracted by a palatable diet .
	manualset3
95388	3	400673	13	NULL	NULL	0	NULL	 thiol content	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the prefrontal cortex , handling reduced thiol content and appears to imbalance the antioxidant enzymes system , which is counteracted by a palatable diet .
	manualset3
95389	4	400673	13	NULL	NULL	0	NULL	imbalance the antioxidant enzymes system	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the prefrontal cortex , handling reduced thiol content and appears to imbalance the antioxidant enzymes system , which is counteracted by a palatable diet .
	manualset3
95390	5	400673	13	NULL	NULL	0	NULL	palatable diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	In the prefrontal cortex , handling reduced thiol content and appears to imbalance the antioxidant enzymes system , which is counteracted by a palatable diet .
	manualset3
95391	1	400674	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of 5-hydroxydeoxycytidine , there was a loss of viral replication after sequential passages of HIV in human CEM cells ( Loeb LA , et al. : Proc Natl Acad Sci USA 1999 ; 96 : 14921497 ) .
	manualset3
95392	2	400674	13	NULL	NULL	0	NULL	5-hydroxydeoxycytidine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of 5-hydroxydeoxycytidine , there was a loss of viral replication after sequential passages of HIV in human CEM cells ( Loeb LA , et al. : Proc Natl Acad Sci USA 1999 ; 96 : 14921497 ) .
	manualset3
95393	3	400674	13	NULL	NULL	0	NULL	loss of viral replication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of 5-hydroxydeoxycytidine , there was a loss of viral replication after sequential passages of HIV in human CEM cells ( Loeb LA , et al. : Proc Natl Acad Sci USA 1999 ; 96 : 14921497 ) .
	manualset3
95394	4	400674	13	NULL	NULL	0	NULL	sequential passages	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of 5-hydroxydeoxycytidine , there was a loss of viral replication after sequential passages of HIV in human CEM cells ( Loeb LA , et al. : Proc Natl Acad Sci USA 1999 ; 96 : 14921497 ) .
	manualset3
95395	5	400674	13	NULL	NULL	0	NULL	HIV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of 5-hydroxydeoxycytidine , there was a loss of viral replication after sequential passages of HIV in human CEM cells ( Loeb LA , et al. : Proc Natl Acad Sci USA 1999 ; 96 : 14921497 ) .
	manualset3
95396	6	400674	13	NULL	NULL	0	NULL	 human CEM cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of 5-hydroxydeoxycytidine , there was a loss of viral replication after sequential passages of HIV in human CEM cells ( Loeb LA , et al. : Proc Natl Acad Sci USA 1999 ; 96 : 14921497 ) .
	manualset3
95397	7	400674	13	NULL	NULL	0	NULL	 Loeb LA 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of 5-hydroxydeoxycytidine , there was a loss of viral replication after sequential passages of HIV in human CEM cells ( Loeb LA , et al. : Proc Natl Acad Sci USA 1999 ; 96 : 14921497 ) .
	manualset3
95398	8	400674	13	NULL	NULL	0	NULL	Proc Natl Acad Sci USA 1999 ; 96 : 14921497 	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of 5-hydroxydeoxycytidine , there was a loss of viral replication after sequential passages of HIV in human CEM cells ( Loeb LA , et al. : Proc Natl Acad Sci USA 1999 ; 96 : 14921497 ) .
	manualset3
95399	1	400675	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of Kv beta 2.1 these values were -14.1 + / - 1.8 and -22.1 + / - 3.7 mV , respectively .
	manualset3
95400	2	400675	13	NULL	NULL	0	NULL	Kv beta 2.1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of Kv beta 2.1 these values were -14.1 + / - 1.8 and -22.1 + / - 3.7 mV , respectively .
	manualset3
95401	3	400675	13	NULL	NULL	NULL	NULL	-14.1 + / - 1.8 mV	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the presence of Kv beta 2.1 these values were -14.1 + / - 1.8 and -22.1 + / - 3.7 mV , respectively .
	manualset3
95402	4	400675	13	NULL	NULL	0	NULL	-22.1 + / - 3.7 mV 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of Kv beta 2.1 these values were -14.1 + / - 1.8 and -22.1 + / - 3.7 mV , respectively .
	manualset3
95403	1	400676	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of L-NOARG ( 0.1 mM ) , electrical field stimulation ( EFS ) induced atropine - and tetrodotoxin-sensitive contractions .
	manualset3
95404	2	400676	13	NULL	NULL	0	NULL	L-NOARG 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of L-NOARG ( 0.1 mM ) , electrical field stimulation ( EFS ) induced atropine - and tetrodotoxin-sensitive contractions .
	manualset3
95405	3	400676	13	NULL	NULL	0	NULL	0.1 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of L-NOARG ( 0.1 mM ) , electrical field stimulation ( EFS ) induced atropine - and tetrodotoxin-sensitive contractions .
	manualset3
95406	4	400676	13	NULL	NULL	0	NULL	electrical field stimulation ( EFS )	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of L-NOARG ( 0.1 mM ) , electrical field stimulation ( EFS ) induced atropine - and tetrodotoxin-sensitive contractions .
	manualset3
95407	5	400676	13	NULL	NULL	0	NULL	atropine-sensitive contractions 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of L-NOARG ( 0.1 mM ) , electrical field stimulation ( EFS ) induced atropine - and tetrodotoxin-sensitive contractions .
	manualset3
95408	6	400676	13	NULL	NULL	0	NULL	tetrodotoxin-sensitive contractions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of L-NOARG ( 0.1 mM ) , electrical field stimulation ( EFS ) induced atropine - and tetrodotoxin-sensitive contractions .
	manualset3
95409	1	400677	13	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of cholecystographic agents or sulfobromophthalein ( BSP ) , the amount of labeled hormone bound to adsorbent increased in a dose-dependent fashion , reflecting displacement from protein-binding sites .
	manualset3
95410	2	400677	13	NULL	NULL	0	NULL	cholecystographic agents	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of cholecystographic agents or sulfobromophthalein ( BSP ) , the amount of labeled hormone bound to adsorbent increased in a dose-dependent fashion , reflecting displacement from protein-binding sites .
	manualset3
95411	3	400677	13	NULL	NULL	0	NULL	sulfobromophthalein ( BSP )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of cholecystographic agents or sulfobromophthalein ( BSP ) , the amount of labeled hormone bound to adsorbent increased in a dose-dependent fashion , reflecting displacement from protein-binding sites .
	manualset3
95412	4	400677	13	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of cholecystographic agents or sulfobromophthalein ( BSP ) , the amount of labeled hormone bound to adsorbent increased in a dose-dependent fashion , reflecting displacement from protein-binding sites .
	manualset3
95413	5	400677	13	NULL	NULL	NULL	NULL	hormone	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the presence of cholecystographic agents or sulfobromophthalein ( BSP ) , the amount of labeled hormone bound to adsorbent increased in a dose-dependent fashion , reflecting displacement from protein-binding sites .
	manualset3
95414	6	400677	13	NULL	NULL	0	NULL	adsorbent 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of cholecystographic agents or sulfobromophthalein ( BSP ) , the amount of labeled hormone bound to adsorbent increased in a dose-dependent fashion , reflecting displacement from protein-binding sites .
	manualset3
95415	7	400677	13	NULL	NULL	0	NULL	dose-dependent fashion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of cholecystographic agents or sulfobromophthalein ( BSP ) , the amount of labeled hormone bound to adsorbent increased in a dose-dependent fashion , reflecting displacement from protein-binding sites .
	manualset3
95416	8	400677	13	NULL	NULL	0	NULL	displacement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of cholecystographic agents or sulfobromophthalein ( BSP ) , the amount of labeled hormone bound to adsorbent increased in a dose-dependent fashion , reflecting displacement from protein-binding sites .
	manualset3
95417	9	400677	13	NULL	NULL	0	NULL	protein-binding sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of cholecystographic agents or sulfobromophthalein ( BSP ) , the amount of labeled hormone bound to adsorbent increased in a dose-dependent fashion , reflecting displacement from protein-binding sites .
	manualset3
95418	1	400678	13	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of l-NAME ( 100M ) the sensitivity and maximum response to CVE were increased , whilst MgSO ( 4 ) ( 6mM ) decreased both parameters .
	manualset3
95419	2	400678	13	NULL	NULL	0	NULL	l-NAME	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of l-NAME ( 100M ) the sensitivity and maximum response to CVE were increased , whilst MgSO ( 4 ) ( 6mM ) decreased both parameters .
	manualset3
95420	3	400678	13	NULL	NULL	0	NULL	100M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of l-NAME ( 100M ) the sensitivity and maximum response to CVE were increased , whilst MgSO ( 4 ) ( 6mM ) decreased both parameters .
	manualset3
95421	4	400678	13	NULL	NULL	0	NULL	sensitivity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of l-NAME ( 100M ) the sensitivity and maximum response to CVE were increased , whilst MgSO ( 4 ) ( 6mM ) decreased both parameters .
	manualset3
95422	5	400678	13	NULL	NULL	NULL	NULL	response 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the presence of l-NAME ( 100M ) the sensitivity and maximum response to CVE were increased , whilst MgSO ( 4 ) ( 6mM ) decreased both parameters .
	manualset3
95423	6	400678	13	NULL	NULL	NULL	NULL	CVE	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the presence of l-NAME ( 100M ) the sensitivity and maximum response to CVE were increased , whilst MgSO ( 4 ) ( 6mM ) decreased both parameters .
	manualset3
95424	7	400678	13	NULL	NULL	NULL	NULL	 MgSO ( 4 ) 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the presence of l-NAME ( 100M ) the sensitivity and maximum response to CVE were increased , whilst MgSO ( 4 ) ( 6mM ) decreased both parameters .
	manualset3
95425	8	400678	13	NULL	NULL	0	NULL	6mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of l-NAME ( 100M ) the sensitivity and maximum response to CVE were increased , whilst MgSO ( 4 ) ( 6mM ) decreased both parameters .
	manualset3
95426	9	400678	13	NULL	NULL	0	NULL	parameters 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of l-NAME ( 100M ) the sensitivity and maximum response to CVE were increased , whilst MgSO ( 4 ) ( 6mM ) decreased both parameters .
	manualset3
95427	1	400679	13	NULL	NULL	0	NULL	presence of liver disease	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of liver disease , heart failure , or serious illness , caution must be applied in theophylline dosing , with frequent monitoring of serum levels .
	manualset3
95428	2	400679	13	NULL	NULL	0	NULL	heart failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of liver disease , heart failure , or serious illness , caution must be applied in theophylline dosing , with frequent monitoring of serum levels .
	manualset3
95429	3	400679	13	NULL	NULL	0	NULL	serious illness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of liver disease , heart failure , or serious illness , caution must be applied in theophylline dosing , with frequent monitoring of serum levels .
	manualset3
95430	4	400679	13	NULL	NULL	0	NULL	caution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of liver disease , heart failure , or serious illness , caution must be applied in theophylline dosing , with frequent monitoring of serum levels .
	manualset3
95431	5	400679	13	NULL	NULL	0	NULL	theophylline dosing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of liver disease , heart failure , or serious illness , caution must be applied in theophylline dosing , with frequent monitoring of serum levels .
	manualset3
95432	6	400679	13	NULL	NULL	0	NULL	frequent monitoring	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of liver disease , heart failure , or serious illness , caution must be applied in theophylline dosing , with frequent monitoring of serum levels .
	manualset3
95433	7	400679	13	NULL	NULL	0	NULL	serum levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of liver disease , heart failure , or serious illness , caution must be applied in theophylline dosing , with frequent monitoring of serum levels .
	manualset3
95434	1	400680	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of ruthenium ( II ) as the maker ion , the behavior of AmB to form ion channels in sterol-free and cholesterol - or ergosterol-containing supported phosphatidylcholine bilayer model membranes were studied by cyclic votammetry , AC impedance spectroscopy , and UV/visible absorbance spectroscopy .
	manualset3
95435	2	400680	13	NULL	NULL	0	NULL	 ruthenium ( II )	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of ruthenium ( II ) as the maker ion , the behavior of AmB to form ion channels in sterol-free and cholesterol - or ergosterol-containing supported phosphatidylcholine bilayer model membranes were studied by cyclic votammetry , AC impedance spectroscopy , and UV/visible absorbance spectroscopy .
	manualset3
95436	3	400680	13	NULL	NULL	0	NULL	maker ion	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of ruthenium ( II ) as the maker ion , the behavior of AmB to form ion channels in sterol-free and cholesterol - or ergosterol-containing supported phosphatidylcholine bilayer model membranes were studied by cyclic votammetry , AC impedance spectroscopy , and UV/visible absorbance spectroscopy .
	manualset3
95437	4	400680	13	NULL	NULL	0	NULL	behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of ruthenium ( II ) as the maker ion , the behavior of AmB to form ion channels in sterol-free and cholesterol - or ergosterol-containing supported phosphatidylcholine bilayer model membranes were studied by cyclic votammetry , AC impedance spectroscopy , and UV/visible absorbance spectroscopy .
	manualset3
95438	5	400680	13	NULL	NULL	0	NULL	AmB 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of ruthenium ( II ) as the maker ion , the behavior of AmB to form ion channels in sterol-free and cholesterol - or ergosterol-containing supported phosphatidylcholine bilayer model membranes were studied by cyclic votammetry , AC impedance spectroscopy , and UV/visible absorbance spectroscopy .
	manualset3
95439	6	400680	13	NULL	NULL	0	NULL	ion channels	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of ruthenium ( II ) as the maker ion , the behavior of AmB to form ion channels in sterol-free and cholesterol - or ergosterol-containing supported phosphatidylcholine bilayer model membranes were studied by cyclic votammetry , AC impedance spectroscopy , and UV/visible absorbance spectroscopy .
	manualset3
95440	7	400680	13	NULL	NULL	0	NULL	sterol-free and cholesterol - or ergosterol-containing supported phosphatidylcholine bilayer model membranes	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of ruthenium ( II ) as the maker ion , the behavior of AmB to form ion channels in sterol-free and cholesterol - or ergosterol-containing supported phosphatidylcholine bilayer model membranes were studied by cyclic votammetry , AC impedance spectroscopy , and UV/visible absorbance spectroscopy .
	manualset3
95441	8	400680	13	NULL	NULL	0	NULL	cyclic votammetry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of ruthenium ( II ) as the maker ion , the behavior of AmB to form ion channels in sterol-free and cholesterol - or ergosterol-containing supported phosphatidylcholine bilayer model membranes were studied by cyclic votammetry , AC impedance spectroscopy , and UV/visible absorbance spectroscopy .
	manualset3
95442	9	400680	13	NULL	NULL	0	NULL	AC impedance spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of ruthenium ( II ) as the maker ion , the behavior of AmB to form ion channels in sterol-free and cholesterol - or ergosterol-containing supported phosphatidylcholine bilayer model membranes were studied by cyclic votammetry , AC impedance spectroscopy , and UV/visible absorbance spectroscopy .
	manualset3
95443	10	400680	13	NULL	NULL	0	NULL	UV/visible absorbance spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of ruthenium ( II ) as the maker ion , the behavior of AmB to form ion channels in sterol-free and cholesterol - or ergosterol-containing supported phosphatidylcholine bilayer model membranes were studied by cyclic votammetry , AC impedance spectroscopy , and UV/visible absorbance spectroscopy .
	manualset3
95444	1	400681	13	NULL	NULL	0	NULL	communication	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present communication the calcium binding proteins responsible for the calcium binding activity peaks resolved by gel permeation chromatography , have been purified and identified as caligulin , ( Mr 40 , 000 ) , calcineurin , ( Mr 230 , 000 ) and calmodulin , ( Mr 38 , 000 ) .
	manualset3
95445	2	400681	13	NULL	NULL	0	NULL	calcium binding proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present communication the calcium binding proteins responsible for the calcium binding activity peaks resolved by gel permeation chromatography , have been purified and identified as caligulin , ( Mr 40 , 000 ) , calcineurin , ( Mr 230 , 000 ) and calmodulin , ( Mr 38 , 000 ) .
	manualset3
95446	3	400681	13	NULL	NULL	NULL	NULL	calcium binding activity peaks	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the present communication the calcium binding proteins responsible for the calcium binding activity peaks resolved by gel permeation chromatography , have been purified and identified as caligulin , ( Mr 40 , 000 ) , calcineurin , ( Mr 230 , 000 ) and calmodulin , ( Mr 38 , 000 ) .
	manualset3
95447	4	400681	13	NULL	NULL	0	NULL	gel permeation chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present communication the calcium binding proteins responsible for the calcium binding activity peaks resolved by gel permeation chromatography , have been purified and identified as caligulin , ( Mr 40 , 000 ) , calcineurin , ( Mr 230 , 000 ) and calmodulin , ( Mr 38 , 000 ) .
	manualset3
95448	5	400681	13	NULL	NULL	0	NULL	caligulin , ( Mr 40 , 000 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present communication the calcium binding proteins responsible for the calcium binding activity peaks resolved by gel permeation chromatography , have been purified and identified as caligulin , ( Mr 40 , 000 ) , calcineurin , ( Mr 230 , 000 ) and calmodulin , ( Mr 38 , 000 ) .
	manualset3
95449	6	400681	13	NULL	NULL	0	NULL	calcineurin , ( Mr 230 , 000 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present communication the calcium binding proteins responsible for the calcium binding activity peaks resolved by gel permeation chromatography , have been purified and identified as caligulin , ( Mr 40 , 000 ) , calcineurin , ( Mr 230 , 000 ) and calmodulin , ( Mr 38 , 000 ) .
	manualset3
95450	7	400681	13	NULL	NULL	0	NULL	 calmodulin , ( Mr 38 , 000 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present communication the calcium binding proteins responsible for the calcium binding activity peaks resolved by gel permeation chromatography , have been purified and identified as caligulin , ( Mr 40 , 000 ) , calcineurin , ( Mr 230 , 000 ) and calmodulin , ( Mr 38 , 000 ) .
	manualset3
95451	1	400682	13	NULL	NULL	0	NULL	present paper	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present paper , features of hyperspectral images are analyzed first in detail , then inter-spectral prediction algorithm is improved , and a new scheme which consists of subspace partition and multi-inter-spectral prediction is proposed , and finally , the experiments show that the program is effective .
	manualset3
95452	2	400682	13	NULL	NULL	0	NULL	features of hyperspectral images 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present paper , features of hyperspectral images are analyzed first in detail , then inter-spectral prediction algorithm is improved , and a new scheme which consists of subspace partition and multi-inter-spectral prediction is proposed , and finally , the experiments show that the program is effective .
	manualset3
95453	3	400682	13	NULL	NULL	0	NULL	detail	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present paper , features of hyperspectral images are analyzed first in detail , then inter-spectral prediction algorithm is improved , and a new scheme which consists of subspace partition and multi-inter-spectral prediction is proposed , and finally , the experiments show that the program is effective .
	manualset3
95454	4	400682	13	NULL	NULL	0	NULL	inter-spectral prediction algorithm	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present paper , features of hyperspectral images are analyzed first in detail , then inter-spectral prediction algorithm is improved , and a new scheme which consists of subspace partition and multi-inter-spectral prediction is proposed , and finally , the experiments show that the program is effective .
	manualset3
95455	5	400682	13	NULL	NULL	0	NULL	new scheme	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present paper , features of hyperspectral images are analyzed first in detail , then inter-spectral prediction algorithm is improved , and a new scheme which consists of subspace partition and multi-inter-spectral prediction is proposed , and finally , the experiments show that the program is effective .
	manualset3
95456	6	400682	13	NULL	NULL	0	NULL	 subspace partition and multi-inter-spectral prediction	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present paper , features of hyperspectral images are analyzed first in detail , then inter-spectral prediction algorithm is improved , and a new scheme which consists of subspace partition and multi-inter-spectral prediction is proposed , and finally , the experiments show that the program is effective .
	manualset3
95457	7	400682	13	NULL	NULL	0	NULL	experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present paper , features of hyperspectral images are analyzed first in detail , then inter-spectral prediction algorithm is improved , and a new scheme which consists of subspace partition and multi-inter-spectral prediction is proposed , and finally , the experiments show that the program is effective .
	manualset3
95458	8	400682	13	NULL	NULL	0	NULL	program	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present paper , features of hyperspectral images are analyzed first in detail , then inter-spectral prediction algorithm is improved , and a new scheme which consists of subspace partition and multi-inter-spectral prediction is proposed , and finally , the experiments show that the program is effective .
	manualset3
95459	1	400683	13	NULL	NULL	0	NULL	report 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present report we show that activation of both purified T lymphocytes and Jurkat cells , through CD43 cross-linking with the anti-CD43 L10 monoclonal antibody , induced CD43 association to Fyn kinase .
	manualset3
95460	2	400683	13	NULL	NULL	0	NULL	 activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present report we show that activation of both purified T lymphocytes and Jurkat cells , through CD43 cross-linking with the anti-CD43 L10 monoclonal antibody , induced CD43 association to Fyn kinase .
	manualset3
95461	3	400683	13	NULL	NULL	0	NULL	T lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present report we show that activation of both purified T lymphocytes and Jurkat cells , through CD43 cross-linking with the anti-CD43 L10 monoclonal antibody , induced CD43 association to Fyn kinase .
	manualset3
95462	4	400683	13	NULL	NULL	0	NULL	Jurkat cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present report we show that activation of both purified T lymphocytes and Jurkat cells , through CD43 cross-linking with the anti-CD43 L10 monoclonal antibody , induced CD43 association to Fyn kinase .
	manualset3
95463	5	400683	13	NULL	NULL	0	NULL	CD43 cross-linking	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present report we show that activation of both purified T lymphocytes and Jurkat cells , through CD43 cross-linking with the anti-CD43 L10 monoclonal antibody , induced CD43 association to Fyn kinase .
	manualset3
95464	6	400683	13	NULL	NULL	0	NULL	anti-CD43 L10 monoclonal antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present report we show that activation of both purified T lymphocytes and Jurkat cells , through CD43 cross-linking with the anti-CD43 L10 monoclonal antibody , induced CD43 association to Fyn kinase .
	manualset3
95465	7	400683	13	NULL	NULL	0	NULL	CD43 association to Fyn kinase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present report we show that activation of both purified T lymphocytes and Jurkat cells , through CD43 cross-linking with the anti-CD43 L10 monoclonal antibody , induced CD43 association to Fyn kinase .
	manualset3
95466	1	400684	13	NULL	NULL	0	NULL	present review	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present review , we summarize recent findings showing that autophagy contributes to the development of the nervous system by providing energy for cell corpse removal after physiological cell death , a process associated with retinal neurogenesis .
	manualset3
95467	2	400684	13	NULL	NULL	0	NULL	recent findings 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present review , we summarize recent findings showing that autophagy contributes to the development of the nervous system by providing energy for cell corpse removal after physiological cell death , a process associated with retinal neurogenesis .
	manualset3
95468	3	400684	13	NULL	NULL	0	NULL	 autophagy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present review , we summarize recent findings showing that autophagy contributes to the development of the nervous system by providing energy for cell corpse removal after physiological cell death , a process associated with retinal neurogenesis .
	manualset3
95469	4	400684	13	NULL	NULL	0	NULL	development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present review , we summarize recent findings showing that autophagy contributes to the development of the nervous system by providing energy for cell corpse removal after physiological cell death , a process associated with retinal neurogenesis .
	manualset3
95470	5	400684	13	NULL	NULL	0	NULL	 nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present review , we summarize recent findings showing that autophagy contributes to the development of the nervous system by providing energy for cell corpse removal after physiological cell death , a process associated with retinal neurogenesis .
	manualset3
95471	6	400684	13	NULL	NULL	0	NULL	energy	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present review , we summarize recent findings showing that autophagy contributes to the development of the nervous system by providing energy for cell corpse removal after physiological cell death , a process associated with retinal neurogenesis .
	manualset3
95472	7	400684	13	NULL	NULL	0	NULL	cell corpse removal	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present review , we summarize recent findings showing that autophagy contributes to the development of the nervous system by providing energy for cell corpse removal after physiological cell death , a process associated with retinal neurogenesis .
	manualset3
95473	8	400684	13	NULL	NULL	0	NULL	physiological cell death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present review , we summarize recent findings showing that autophagy contributes to the development of the nervous system by providing energy for cell corpse removal after physiological cell death , a process associated with retinal neurogenesis .
	manualset3
95474	9	400684	13	NULL	NULL	0	NULL	process	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present review , we summarize recent findings showing that autophagy contributes to the development of the nervous system by providing energy for cell corpse removal after physiological cell death , a process associated with retinal neurogenesis .
	manualset3
95475	10	400684	13	NULL	NULL	0	NULL	 retinal neurogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present review , we summarize recent findings showing that autophagy contributes to the development of the nervous system by providing energy for cell corpse removal after physiological cell death , a process associated with retinal neurogenesis .
	manualset3
95476	1	400685	13	NULL	NULL	0	NULL	present review article 	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present review article the pathophysiology of the relevant valvular heart diseases and the implications for perioperative anesthesia management will be presented .
	manualset3
95477	2	400685	13	NULL	NULL	0	NULL	 pathophysiology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present review article the pathophysiology of the relevant valvular heart diseases and the implications for perioperative anesthesia management will be presented .
	manualset3
95478	3	400685	13	NULL	NULL	0	NULL	valvular heart diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present review article the pathophysiology of the relevant valvular heart diseases and the implications for perioperative anesthesia management will be presented .
	manualset3
95479	4	400685	13	NULL	NULL	0	NULL	implications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present review article the pathophysiology of the relevant valvular heart diseases and the implications for perioperative anesthesia management will be presented .
	manualset3
95480	5	400685	13	NULL	NULL	0	NULL	perioperative anesthesia management 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present review article the pathophysiology of the relevant valvular heart diseases and the implications for perioperative anesthesia management will be presented .
	manualset3
95481	1	400686	13	NULL	NULL	0	NULL	present studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present studies , we have employed a novel mutagenesis-based approach to identify the macromolecular determinants that control H4 N-terminal domain ( NTD ) function during oligomerization .
	manualset3
95482	2	400686	13	NULL	NULL	0	NULL	novel mutagenesis-based approach 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present studies , we have employed a novel mutagenesis-based approach to identify the macromolecular determinants that control H4 N-terminal domain ( NTD ) function during oligomerization .
	manualset3
95483	3	400686	13	NULL	NULL	0	NULL	macromolecular determinants	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present studies , we have employed a novel mutagenesis-based approach to identify the macromolecular determinants that control H4 N-terminal domain ( NTD ) function during oligomerization .
	manualset3
95484	4	400686	13	NULL	NULL	0	NULL	H4 N-terminal domain ( NTD ) function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present studies , we have employed a novel mutagenesis-based approach to identify the macromolecular determinants that control H4 N-terminal domain ( NTD ) function during oligomerization .
	manualset3
95485	5	400686	13	NULL	NULL	0	NULL	oligomerization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present studies , we have employed a novel mutagenesis-based approach to identify the macromolecular determinants that control H4 N-terminal domain ( NTD ) function during oligomerization .
	manualset3
95486	1	400687	13	NULL	NULL	0	NULL	present studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present studies inheritance of the characteristic light chain patterns has been studied in the AKXL recombinant inbred lines ( derived from C57L/J and AKR/J parental lines ) and in the inbred Ly-2a , 3 a congenic line B6.PL-Ly-2aLy-3a / Cy as well as in individual backcross animals of an incipient Ly-2a , 3 a congenic strain .
	manualset3
95487	2	400687	13	NULL	NULL	0	NULL	inheritance of the characteristic light chain patterns 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present studies inheritance of the characteristic light chain patterns has been studied in the AKXL recombinant inbred lines ( derived from C57L/J and AKR/J parental lines ) and in the inbred Ly-2a , 3 a congenic line B6.PL-Ly-2aLy-3a / Cy as well as in individual backcross animals of an incipient Ly-2a , 3 a congenic strain .
	manualset3
95488	3	400687	13	NULL	NULL	0	NULL	AKXL recombinant inbred lines 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present studies inheritance of the characteristic light chain patterns has been studied in the AKXL recombinant inbred lines ( derived from C57L/J and AKR/J parental lines ) and in the inbred Ly-2a , 3 a congenic line B6.PL-Ly-2aLy-3a / Cy as well as in individual backcross animals of an incipient Ly-2a , 3 a congenic strain .
	manualset3
95489	4	400687	13	NULL	NULL	0	NULL	C57L/J parental line	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present studies inheritance of the characteristic light chain patterns has been studied in the AKXL recombinant inbred lines ( derived from C57L/J and AKR/J parental lines ) and in the inbred Ly-2a , 3 a congenic line B6.PL-Ly-2aLy-3a / Cy as well as in individual backcross animals of an incipient Ly-2a , 3 a congenic strain .
	manualset3
95490	5	400687	13	NULL	NULL	0	NULL	AKR/J parental line	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present studies inheritance of the characteristic light chain patterns has been studied in the AKXL recombinant inbred lines ( derived from C57L/J and AKR/J parental lines ) and in the inbred Ly-2a , 3 a congenic line B6.PL-Ly-2aLy-3a / Cy as well as in individual backcross animals of an incipient Ly-2a , 3 a congenic strain .
	manualset3
95491	6	400687	13	NULL	NULL	0	NULL	inbred Ly-2a , 3 a congenic line B6.PL-Ly-2aLy-3a / Cy 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present studies inheritance of the characteristic light chain patterns has been studied in the AKXL recombinant inbred lines ( derived from C57L/J and AKR/J parental lines ) and in the inbred Ly-2a , 3 a congenic line B6.PL-Ly-2aLy-3a / Cy as well as in individual backcross animals of an incipient Ly-2a , 3 a congenic strain .
	manualset3
95492	7	400687	13	NULL	NULL	0	NULL	individual backcross animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present studies inheritance of the characteristic light chain patterns has been studied in the AKXL recombinant inbred lines ( derived from C57L/J and AKR/J parental lines ) and in the inbred Ly-2a , 3 a congenic line B6.PL-Ly-2aLy-3a / Cy as well as in individual backcross animals of an incipient Ly-2a , 3 a congenic strain .
	manualset3
95493	8	400687	13	NULL	NULL	0	NULL	incipient Ly-2a , 3 a congenic strain 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present studies inheritance of the characteristic light chain patterns has been studied in the AKXL recombinant inbred lines ( derived from C57L/J and AKR/J parental lines ) and in the inbred Ly-2a , 3 a congenic line B6.PL-Ly-2aLy-3a / Cy as well as in individual backcross animals of an incipient Ly-2a , 3 a congenic strain .
	manualset3
95494	1	400688	13	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , a recombinant mammalian expression system has been used to study the molecular signals that direct removal of this basic amino acid pair .
	manualset3
95495	2	400688	13	NULL	NULL	0	NULL	recombinant mammalian expression system	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , a recombinant mammalian expression system has been used to study the molecular signals that direct removal of this basic amino acid pair .
	manualset3
95496	3	400688	13	NULL	NULL	0	NULL	molecular signals 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , a recombinant mammalian expression system has been used to study the molecular signals that direct removal of this basic amino acid pair .
	manualset3
95497	4	400688	13	NULL	NULL	0	NULL	removal of this basic amino acid pair	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , a recombinant mammalian expression system has been used to study the molecular signals that direct removal of this basic amino acid pair .
	manualset3
95498	1	400689	13	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , by using data generated from hundreds of mtDNA sequences , we revalue the deuterostome phylogeny in terms of whole mitochondrial genomes ( mitogenomes ) .
	manualset3
95499	2	400689	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , by using data generated from hundreds of mtDNA sequences , we revalue the deuterostome phylogeny in terms of whole mitochondrial genomes ( mitogenomes ) .
	manualset3
95500	3	400689	13	NULL	NULL	0	NULL	hundreds of mtDNA sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , by using data generated from hundreds of mtDNA sequences , we revalue the deuterostome phylogeny in terms of whole mitochondrial genomes ( mitogenomes ) .
	manualset3
95501	4	400689	13	NULL	NULL	0	NULL	deuterostome phylogeny	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , by using data generated from hundreds of mtDNA sequences , we revalue the deuterostome phylogeny in terms of whole mitochondrial genomes ( mitogenomes ) .
	manualset3
95502	5	400689	13	NULL	NULL	0	NULL	mitochondrial genomes ( mitogenomes ) 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , by using data generated from hundreds of mtDNA sequences , we revalue the deuterostome phylogeny in terms of whole mitochondrial genomes ( mitogenomes ) .
	manualset3
95503	1	400690	13	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , dexamethasone-succinate-dextran and dexamethasone-glutarate-dextran were administered to two groups of male Sprague-Dawley rats by intragastric infusion .
	manualset3
95504	2	400690	13	NULL	NULL	0	NULL	dexamethasone-succinate-dextran	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , dexamethasone-succinate-dextran and dexamethasone-glutarate-dextran were administered to two groups of male Sprague-Dawley rats by intragastric infusion .
	manualset3
95505	3	400690	13	NULL	NULL	0	NULL	dexamethasone-glutarate-dextran	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , dexamethasone-succinate-dextran and dexamethasone-glutarate-dextran were administered to two groups of male Sprague-Dawley rats by intragastric infusion .
	manualset3
95506	4	400690	13	NULL	NULL	0	NULL	two groups	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , dexamethasone-succinate-dextran and dexamethasone-glutarate-dextran were administered to two groups of male Sprague-Dawley rats by intragastric infusion .
	manualset3
95507	5	400690	13	NULL	NULL	0	NULL	male Sprague-Dawley rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , dexamethasone-succinate-dextran and dexamethasone-glutarate-dextran were administered to two groups of male Sprague-Dawley rats by intragastric infusion .
	manualset3
95508	6	400690	13	NULL	NULL	0	NULL	intragastric infusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , dexamethasone-succinate-dextran and dexamethasone-glutarate-dextran were administered to two groups of male Sprague-Dawley rats by intragastric infusion .
	manualset3
95509	1	400691	13	NULL	NULL	0	NULL	 present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , line blot analyses were performed using recombinant complement regulator-acquiring surface protein 2 ( BbCRASP-2 ) from Borrelia burgdorferi sensu stricto strain B31 and serum samples from human Lyme disease patients from throughout the United States and Germany .
	manualset3
95510	2	400691	13	NULL	NULL	0	NULL	line blot analyses 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , line blot analyses were performed using recombinant complement regulator-acquiring surface protein 2 ( BbCRASP-2 ) from Borrelia burgdorferi sensu stricto strain B31 and serum samples from human Lyme disease patients from throughout the United States and Germany .
	manualset3
95511	3	400691	13	NULL	NULL	0	NULL	recombinant complement regulator-acquiring surface protein 2 ( BbCRASP-2 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , line blot analyses were performed using recombinant complement regulator-acquiring surface protein 2 ( BbCRASP-2 ) from Borrelia burgdorferi sensu stricto strain B31 and serum samples from human Lyme disease patients from throughout the United States and Germany .
	manualset3
95512	4	400691	13	NULL	NULL	0	NULL	Borrelia burgdorferi sensu stricto strain B31 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , line blot analyses were performed using recombinant complement regulator-acquiring surface protein 2 ( BbCRASP-2 ) from Borrelia burgdorferi sensu stricto strain B31 and serum samples from human Lyme disease patients from throughout the United States and Germany .
	manualset3
95513	5	400691	13	NULL	NULL	0	NULL	serum samples 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , line blot analyses were performed using recombinant complement regulator-acquiring surface protein 2 ( BbCRASP-2 ) from Borrelia burgdorferi sensu stricto strain B31 and serum samples from human Lyme disease patients from throughout the United States and Germany .
	manualset3
95514	6	400691	13	NULL	NULL	0	NULL	human Lyme disease patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , line blot analyses were performed using recombinant complement regulator-acquiring surface protein 2 ( BbCRASP-2 ) from Borrelia burgdorferi sensu stricto strain B31 and serum samples from human Lyme disease patients from throughout the United States and Germany .
	manualset3
95515	7	400691	13	NULL	NULL	0	NULL	United States	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , line blot analyses were performed using recombinant complement regulator-acquiring surface protein 2 ( BbCRASP-2 ) from Borrelia burgdorferi sensu stricto strain B31 and serum samples from human Lyme disease patients from throughout the United States and Germany .
	manualset3
95516	8	400691	13	NULL	NULL	0	NULL	 Germany	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , line blot analyses were performed using recombinant complement regulator-acquiring surface protein 2 ( BbCRASP-2 ) from Borrelia burgdorferi sensu stricto strain B31 and serum samples from human Lyme disease patients from throughout the United States and Germany .
	manualset3
95517	1	400692	13	NULL	NULL	0	NULL	10 ( 4 ) parasites	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	10 ( 4 ) parasites were used , except in the case of IM treatment , where mice received 10 ( 3 ) trypomastigotes in one group and 10 ( 5 ) in another .
	manualset3
95518	2	400692	13	NULL	NULL	0	NULL	case of IM treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	10 ( 4 ) parasites were used , except in the case of IM treatment , where mice received 10 ( 3 ) trypomastigotes in one group and 10 ( 5 ) in another .
	manualset3
95519	3	400692	13	NULL	NULL	0	NULL	mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	10 ( 4 ) parasites were used , except in the case of IM treatment , where mice received 10 ( 3 ) trypomastigotes in one group and 10 ( 5 ) in another .
	manualset3
95520	4	400692	13	NULL	NULL	0	NULL	10 ( 3 ) trypomastigotes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	10 ( 4 ) parasites were used , except in the case of IM treatment , where mice received 10 ( 3 ) trypomastigotes in one group and 10 ( 5 ) in another .
	manualset3
95521	5	400692	13	NULL	NULL	0	NULL	one group 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	10 ( 4 ) parasites were used , except in the case of IM treatment , where mice received 10 ( 3 ) trypomastigotes in one group and 10 ( 5 ) in another .
	manualset3
95522	6	400692	13	NULL	NULL	NULL	NULL	10 ( 5 ) trypomastigotes	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	10 ( 4 ) parasites were used , except in the case of IM treatment , where mice received 10 ( 3 ) trypomastigotes in one group and 10 ( 5 ) in another .
	manualset3
95523	1	400693	13	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , ovariectomized female rats were given two injections , 24 h apart , of sesame oil ( control ) , 10 microg EB , 500 microg TP or 500 microg DHT .
	manualset3
95524	2	400693	13	NULL	NULL	0	NULL	ovariectomized female rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , ovariectomized female rats were given two injections , 24 h apart , of sesame oil ( control ) , 10 microg EB , 500 microg TP or 500 microg DHT .
	manualset3
95525	3	400693	13	NULL	NULL	0	NULL	two injections	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , ovariectomized female rats were given two injections , 24 h apart , of sesame oil ( control ) , 10 microg EB , 500 microg TP or 500 microg DHT .
	manualset3
95526	4	400693	13	NULL	NULL	0	NULL	24 h apart	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , ovariectomized female rats were given two injections , 24 h apart , of sesame oil ( control ) , 10 microg EB , 500 microg TP or 500 microg DHT .
	manualset3
95527	5	400693	13	NULL	NULL	0	NULL	sesame oil 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , ovariectomized female rats were given two injections , 24 h apart , of sesame oil ( control ) , 10 microg EB , 500 microg TP or 500 microg DHT .
	manualset3
95528	6	400693	13	NULL	NULL	0	NULL	10 microg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , ovariectomized female rats were given two injections , 24 h apart , of sesame oil ( control ) , 10 microg EB , 500 microg TP or 500 microg DHT .
	manualset3
95529	7	400693	13	NULL	NULL	0	NULL	EB	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , ovariectomized female rats were given two injections , 24 h apart , of sesame oil ( control ) , 10 microg EB , 500 microg TP or 500 microg DHT .
	manualset3
95530	8	400693	13	NULL	NULL	0	NULL	500 microg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , ovariectomized female rats were given two injections , 24 h apart , of sesame oil ( control ) , 10 microg EB , 500 microg TP or 500 microg DHT .
	manualset3
95531	9	400693	13	NULL	NULL	0	NULL	TP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , ovariectomized female rats were given two injections , 24 h apart , of sesame oil ( control ) , 10 microg EB , 500 microg TP or 500 microg DHT .
	manualset3
95532	10	400693	13	NULL	NULL	0	NULL	500 microg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , ovariectomized female rats were given two injections , 24 h apart , of sesame oil ( control ) , 10 microg EB , 500 microg TP or 500 microg DHT .
	manualset3
95533	11	400693	13	NULL	NULL	0	NULL	DHT 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , ovariectomized female rats were given two injections , 24 h apart , of sesame oil ( control ) , 10 microg EB , 500 microg TP or 500 microg DHT .
	manualset3
95534	1	400694	13	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , several putative Francisella tularensis glycoproteins were characterized through the combination of carbohydrate-specific detection and lectin affinity with highly sensitive mass spectrometry utilizing the bottom-up proteomic approach .
	manualset3
95535	2	400694	13	NULL	NULL	0	NULL	putative Francisella tularensis glycoproteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , several putative Francisella tularensis glycoproteins were characterized through the combination of carbohydrate-specific detection and lectin affinity with highly sensitive mass spectrometry utilizing the bottom-up proteomic approach .
	manualset3
95536	3	400694	13	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , several putative Francisella tularensis glycoproteins were characterized through the combination of carbohydrate-specific detection and lectin affinity with highly sensitive mass spectrometry utilizing the bottom-up proteomic approach .
	manualset3
95537	4	400694	13	NULL	NULL	0	NULL	carbohydrate-specific detection 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , several putative Francisella tularensis glycoproteins were characterized through the combination of carbohydrate-specific detection and lectin affinity with highly sensitive mass spectrometry utilizing the bottom-up proteomic approach .
	manualset3
95538	5	400694	13	NULL	NULL	0	NULL	lectin affinity	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , several putative Francisella tularensis glycoproteins were characterized through the combination of carbohydrate-specific detection and lectin affinity with highly sensitive mass spectrometry utilizing the bottom-up proteomic approach .
	manualset3
95539	6	400694	13	NULL	NULL	0	NULL	mass spectrometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , several putative Francisella tularensis glycoproteins were characterized through the combination of carbohydrate-specific detection and lectin affinity with highly sensitive mass spectrometry utilizing the bottom-up proteomic approach .
	manualset3
95540	7	400694	13	NULL	NULL	0	NULL	proteomic approach	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , several putative Francisella tularensis glycoproteins were characterized through the combination of carbohydrate-specific detection and lectin affinity with highly sensitive mass spectrometry utilizing the bottom-up proteomic approach .
	manualset3
95541	1	400695	13	NULL	NULL	0	NULL	present study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the N195-Sc fusion protein was highly expressed in insect ( Sf9 ) cells infected with a recombinant baculovirus bearing the hybrid gene under the control of a polyhedrin promoter .
	manualset3
95542	2	400695	13	NULL	NULL	0	NULL	N195-Sc fusion protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the N195-Sc fusion protein was highly expressed in insect ( Sf9 ) cells infected with a recombinant baculovirus bearing the hybrid gene under the control of a polyhedrin promoter .
	manualset3
95543	3	400695	13	NULL	NULL	0	NULL	insect ( Sf9 ) cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the N195-Sc fusion protein was highly expressed in insect ( Sf9 ) cells infected with a recombinant baculovirus bearing the hybrid gene under the control of a polyhedrin promoter .
	manualset3
95544	4	400695	13	NULL	NULL	NULL	NULL	recombinant baculovirus 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the present study , the N195-Sc fusion protein was highly expressed in insect ( Sf9 ) cells infected with a recombinant baculovirus bearing the hybrid gene under the control of a polyhedrin promoter .
	manualset3
95545	7	400695	13	NULL	NULL	NULL	NULL	polyhedrin promoter 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the present study , the N195-Sc fusion protein was highly expressed in insect ( Sf9 ) cells infected with a recombinant baculovirus bearing the hybrid gene under the control of a polyhedrin promoter .
	manualset3
95546	5	400695	13	NULL	NULL	0	NULL	 hybrid gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the N195-Sc fusion protein was highly expressed in insect ( Sf9 ) cells infected with a recombinant baculovirus bearing the hybrid gene under the control of a polyhedrin promoter .
	manualset3
95547	6	400695	13	NULL	NULL	0	NULL	 control 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the N195-Sc fusion protein was highly expressed in insect ( Sf9 ) cells infected with a recombinant baculovirus bearing the hybrid gene under the control of a polyhedrin promoter .
	manualset3
95548	1	400696	13	NULL	NULL	0	NULL	present study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the authors postulated that inhibition of myristoylated alanine-rich C kinase substrate ( MARCKS ) , an 82-kDa protein with multiple biological roles , could inhibit ozone-induced leukocyte trafficking and cytokine secretions .
	manualset3
95549	2	400696	13	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the authors postulated that inhibition of myristoylated alanine-rich C kinase substrate ( MARCKS ) , an 82-kDa protein with multiple biological roles , could inhibit ozone-induced leukocyte trafficking and cytokine secretions .
	manualset3
95550	3	400696	13	NULL	NULL	0	NULL	 inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the authors postulated that inhibition of myristoylated alanine-rich C kinase substrate ( MARCKS ) , an 82-kDa protein with multiple biological roles , could inhibit ozone-induced leukocyte trafficking and cytokine secretions .
	manualset3
95551	4	400696	13	NULL	NULL	0	NULL	myristoylated alanine-rich C kinase substrate ( MARCKS ) , an 82-kDa protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the authors postulated that inhibition of myristoylated alanine-rich C kinase substrate ( MARCKS ) , an 82-kDa protein with multiple biological roles , could inhibit ozone-induced leukocyte trafficking and cytokine secretions .
	manualset3
95552	5	400696	13	NULL	NULL	NULL	NULL	multiple biological roles	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the present study , the authors postulated that inhibition of myristoylated alanine-rich C kinase substrate ( MARCKS ) , an 82-kDa protein with multiple biological roles , could inhibit ozone-induced leukocyte trafficking and cytokine secretions .
	manualset3
95553	6	400696	13	NULL	NULL	NULL	NULL	ozone-induced leukocyte trafficking	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the present study , the authors postulated that inhibition of myristoylated alanine-rich C kinase substrate ( MARCKS ) , an 82-kDa protein with multiple biological roles , could inhibit ozone-induced leukocyte trafficking and cytokine secretions .
	manualset3
95554	7	400696	13	NULL	NULL	0	NULL	cytokine secretions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the authors postulated that inhibition of myristoylated alanine-rich C kinase substrate ( MARCKS ) , an 82-kDa protein with multiple biological roles , could inhibit ozone-induced leukocyte trafficking and cytokine secretions .
	manualset3
95555	1	400697	13	NULL	NULL	0	NULL	 present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the extent of antioxidant protection by nisoldipine against combined NO / * O ( 2 ) ( - ) or peroxynitrite-mediated EC injury was assessed and compared with nicardipine , nifedipine and Trolox ( water-soluble vitamin E ) .
	manualset3
95556	2	400697	13	NULL	NULL	0	NULL	extent of antioxidant protection 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the extent of antioxidant protection by nisoldipine against combined NO / * O ( 2 ) ( - ) or peroxynitrite-mediated EC injury was assessed and compared with nicardipine , nifedipine and Trolox ( water-soluble vitamin E ) .
	manualset3
95557	3	400697	13	NULL	NULL	0	NULL	nisoldipine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the extent of antioxidant protection by nisoldipine against combined NO / * O ( 2 ) ( - ) or peroxynitrite-mediated EC injury was assessed and compared with nicardipine , nifedipine and Trolox ( water-soluble vitamin E ) .
	manualset3
95558	4	400697	13	NULL	NULL	0	NULL	NO / * O ( 2 ) ( - ) or peroxynitrite-mediated EC injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the extent of antioxidant protection by nisoldipine against combined NO / * O ( 2 ) ( - ) or peroxynitrite-mediated EC injury was assessed and compared with nicardipine , nifedipine and Trolox ( water-soluble vitamin E ) .
	manualset3
95559	5	400697	13	NULL	NULL	0	NULL	nicardipine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the extent of antioxidant protection by nisoldipine against combined NO / * O ( 2 ) ( - ) or peroxynitrite-mediated EC injury was assessed and compared with nicardipine , nifedipine and Trolox ( water-soluble vitamin E ) .
	manualset3
95560	6	400697	13	NULL	NULL	0	NULL	nifedipine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the extent of antioxidant protection by nisoldipine against combined NO / * O ( 2 ) ( - ) or peroxynitrite-mediated EC injury was assessed and compared with nicardipine , nifedipine and Trolox ( water-soluble vitamin E ) .
	manualset3
95561	7	400697	13	NULL	NULL	0	NULL	Trolox ( water-soluble vitamin E )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the extent of antioxidant protection by nisoldipine against combined NO / * O ( 2 ) ( - ) or peroxynitrite-mediated EC injury was assessed and compared with nicardipine , nifedipine and Trolox ( water-soluble vitamin E ) .
	manualset3
95562	1	400698	13	NULL	NULL	0	NULL	present study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the in vivo effects of a promising hypoxic cytotoxin , tirapazamine ( 3-amino-1 , 2 , 4 - benzotriazine 1 , 4-di-N-oxide ) , were examined in comparison with those of KU-2285 , one of the best hypoxic cell radiosensitizers , in combination with both single and fractionated irradiation .
	manualset3
95563	2	400698	13	NULL	NULL	0	NULL	 in vivo effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the in vivo effects of a promising hypoxic cytotoxin , tirapazamine ( 3-amino-1 , 2 , 4 - benzotriazine 1 , 4-di-N-oxide ) , were examined in comparison with those of KU-2285 , one of the best hypoxic cell radiosensitizers , in combination with both single and fractionated irradiation .
	manualset3
95564	3	400698	13	NULL	NULL	0	NULL	hypoxic cytotoxin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the in vivo effects of a promising hypoxic cytotoxin , tirapazamine ( 3-amino-1 , 2 , 4 - benzotriazine 1 , 4-di-N-oxide ) , were examined in comparison with those of KU-2285 , one of the best hypoxic cell radiosensitizers , in combination with both single and fractionated irradiation .
	manualset3
95565	4	400698	13	NULL	NULL	0	NULL	 tirapazamine ( 3-amino-1 , 2 , 4 - benzotriazine 1 , 4-di-N-oxide ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the in vivo effects of a promising hypoxic cytotoxin , tirapazamine ( 3-amino-1 , 2 , 4 - benzotriazine 1 , 4-di-N-oxide ) , were examined in comparison with those of KU-2285 , one of the best hypoxic cell radiosensitizers , in combination with both single and fractionated irradiation .
	manualset3
95566	5	400698	13	NULL	NULL	0	NULL	comparison 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the in vivo effects of a promising hypoxic cytotoxin , tirapazamine ( 3-amino-1 , 2 , 4 - benzotriazine 1 , 4-di-N-oxide ) , were examined in comparison with those of KU-2285 , one of the best hypoxic cell radiosensitizers , in combination with both single and fractionated irradiation .
	manualset3
95567	6	400698	13	NULL	NULL	0	NULL	KU-2285 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the in vivo effects of a promising hypoxic cytotoxin , tirapazamine ( 3-amino-1 , 2 , 4 - benzotriazine 1 , 4-di-N-oxide ) , were examined in comparison with those of KU-2285 , one of the best hypoxic cell radiosensitizers , in combination with both single and fractionated irradiation .
	manualset3
95568	7	400698	13	NULL	NULL	0	NULL	hypoxic cell radiosensitizers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the in vivo effects of a promising hypoxic cytotoxin , tirapazamine ( 3-amino-1 , 2 , 4 - benzotriazine 1 , 4-di-N-oxide ) , were examined in comparison with those of KU-2285 , one of the best hypoxic cell radiosensitizers , in combination with both single and fractionated irradiation .
	manualset3
95569	8	400698	13	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the in vivo effects of a promising hypoxic cytotoxin , tirapazamine ( 3-amino-1 , 2 , 4 - benzotriazine 1 , 4-di-N-oxide ) , were examined in comparison with those of KU-2285 , one of the best hypoxic cell radiosensitizers , in combination with both single and fractionated irradiation .
	manualset3
95570	9	400698	13	NULL	NULL	NULL	NULL	single irradiation	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the present study , the in vivo effects of a promising hypoxic cytotoxin , tirapazamine ( 3-amino-1 , 2 , 4 - benzotriazine 1 , 4-di-N-oxide ) , were examined in comparison with those of KU-2285 , one of the best hypoxic cell radiosensitizers , in combination with both single and fractionated irradiation .
	manualset3
98584	10	400698	13	NULL	NULL	0	NULL	fractionated irradiation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the in vivo effects of a promising hypoxic cytotoxin , tirapazamine ( 3-amino-1 , 2 , 4 - benzotriazine 1 , 4-di-N-oxide ) , were examined in comparison with those of KU-2285 , one of the best hypoxic cell radiosensitizers , in combination with both single and fractionated irradiation .
	manualset3
95571	1	400699	13	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the susceptibility of strains CAF2-1 , SSK21 , and SSK23 to killing by human polymorphonuclear neutrophils ( PMNs ) was assessed .
	manualset3
95572	2	400699	13	NULL	NULL	NULL	NULL	susceptibility of strains	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the present study , the susceptibility of strains CAF2-1 , SSK21 , and SSK23 to killing by human polymorphonuclear neutrophils ( PMNs ) was assessed .
	manualset3
95573	3	400699	13	NULL	NULL	0	NULL	CAF2-1 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the susceptibility of strains CAF2-1 , SSK21 , and SSK23 to killing by human polymorphonuclear neutrophils ( PMNs ) was assessed .
	manualset3
95574	4	400699	13	NULL	NULL	0	NULL	SSK21	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the susceptibility of strains CAF2-1 , SSK21 , and SSK23 to killing by human polymorphonuclear neutrophils ( PMNs ) was assessed .
	manualset3
95575	5	400699	13	NULL	NULL	0	NULL	SSK23	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the susceptibility of strains CAF2-1 , SSK21 , and SSK23 to killing by human polymorphonuclear neutrophils ( PMNs ) was assessed .
	manualset3
95576	6	400699	13	NULL	NULL	0	NULL	killing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the susceptibility of strains CAF2-1 , SSK21 , and SSK23 to killing by human polymorphonuclear neutrophils ( PMNs ) was assessed .
	manualset3
95577	7	400699	13	NULL	NULL	0	NULL	human polymorphonuclear neutrophils ( PMNs )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , the susceptibility of strains CAF2-1 , SSK21 , and SSK23 to killing by human polymorphonuclear neutrophils ( PMNs ) was assessed .
	manualset3
95578	1	400700	13	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , these observations have been extended to two pleural models of immune-driven inflammation in the rat , an immediate type III hypersensitivity ( Arthus ) reaction and a delayed type IV hypersensitivity reaction .
	manualset3
95579	2	400700	13	NULL	NULL	0	NULL	observations 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , these observations have been extended to two pleural models of immune-driven inflammation in the rat , an immediate type III hypersensitivity ( Arthus ) reaction and a delayed type IV hypersensitivity reaction .
	manualset3
95580	3	400700	13	NULL	NULL	0	NULL	two pleural models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , these observations have been extended to two pleural models of immune-driven inflammation in the rat , an immediate type III hypersensitivity ( Arthus ) reaction and a delayed type IV hypersensitivity reaction .
	manualset3
95581	4	400700	13	NULL	NULL	0	NULL	immune-driven inflammation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , these observations have been extended to two pleural models of immune-driven inflammation in the rat , an immediate type III hypersensitivity ( Arthus ) reaction and a delayed type IV hypersensitivity reaction .
	manualset3
95582	5	400700	13	NULL	NULL	0	NULL	rat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , these observations have been extended to two pleural models of immune-driven inflammation in the rat , an immediate type III hypersensitivity ( Arthus ) reaction and a delayed type IV hypersensitivity reaction .
	manualset3
95583	6	400700	13	NULL	NULL	0	NULL	type III hypersensitivity ( Arthus ) reaction 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , these observations have been extended to two pleural models of immune-driven inflammation in the rat , an immediate type III hypersensitivity ( Arthus ) reaction and a delayed type IV hypersensitivity reaction .
	manualset3
95584	7	400700	13	NULL	NULL	0	NULL	type IV hypersensitivity reaction 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , these observations have been extended to two pleural models of immune-driven inflammation in the rat , an immediate type III hypersensitivity ( Arthus ) reaction and a delayed type IV hypersensitivity reaction .
	manualset3
95585	1	400701	13	NULL	NULL	0	NULL	 present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we addressed the question of which type of hybrid joining occurs in a physiological environment , where standard V ( D ) J recombination presumably occurs and normal RAG proteins are endogenously expressed .
	manualset3
95586	2	400701	13	NULL	NULL	0	NULL	question	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we addressed the question of which type of hybrid joining occurs in a physiological environment , where standard V ( D ) J recombination presumably occurs and normal RAG proteins are endogenously expressed .
	manualset3
95587	3	400701	13	NULL	NULL	NULL	NULL	 type of hybrid joining 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the present study , we addressed the question of which type of hybrid joining occurs in a physiological environment , where standard V ( D ) J recombination presumably occurs and normal RAG proteins are endogenously expressed .
	manualset3
95588	4	400701	13	NULL	NULL	0	NULL	physiological environment	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we addressed the question of which type of hybrid joining occurs in a physiological environment , where standard V ( D ) J recombination presumably occurs and normal RAG proteins are endogenously expressed .
	manualset3
95589	5	400701	13	NULL	NULL	0	NULL	standard V ( D ) J recombination	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we addressed the question of which type of hybrid joining occurs in a physiological environment , where standard V ( D ) J recombination presumably occurs and normal RAG proteins are endogenously expressed .
	manualset3
95590	6	400701	13	NULL	NULL	0	NULL	RAG proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we addressed the question of which type of hybrid joining occurs in a physiological environment , where standard V ( D ) J recombination presumably occurs and normal RAG proteins are endogenously expressed .
	manualset3
95591	1	400702	13	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we characterize the nature , mode of function , and specificity of the effector cells in this immunity .
	manualset3
95592	2	400702	13	NULL	NULL	0	NULL	 nature	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we characterize the nature , mode of function , and specificity of the effector cells in this immunity .
	manualset3
95593	3	400702	13	NULL	NULL	0	NULL	mode of function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we characterize the nature , mode of function , and specificity of the effector cells in this immunity .
	manualset3
95594	4	400702	13	NULL	NULL	0	NULL	specificity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we characterize the nature , mode of function , and specificity of the effector cells in this immunity .
	manualset3
95595	5	400702	13	NULL	NULL	0	NULL	effector cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we characterize the nature , mode of function , and specificity of the effector cells in this immunity .
	manualset3
95596	6	400702	13	NULL	NULL	0	NULL	immunity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we characterize the nature , mode of function , and specificity of the effector cells in this immunity .
	manualset3
95597	1	400703	13	NULL	NULL	0	NULL	present study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we competed in-vitro transcription of circular template DNA with linear DNA fragments to identify promoter domains responsible for binding and sequestering essential trans-acting transcription factors .
	manualset3
95598	2	400703	13	NULL	NULL	0	NULL	in-vitro transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we competed in-vitro transcription of circular template DNA with linear DNA fragments to identify promoter domains responsible for binding and sequestering essential trans-acting transcription factors .
	manualset3
95599	3	400703	13	NULL	NULL	0	NULL	circular template DNA with linear DNA fragments	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we competed in-vitro transcription of circular template DNA with linear DNA fragments to identify promoter domains responsible for binding and sequestering essential trans-acting transcription factors .
	manualset3
95600	4	400703	13	NULL	NULL	0	NULL	promoter domains 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we competed in-vitro transcription of circular template DNA with linear DNA fragments to identify promoter domains responsible for binding and sequestering essential trans-acting transcription factors .
	manualset3
95601	5	400703	13	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we competed in-vitro transcription of circular template DNA with linear DNA fragments to identify promoter domains responsible for binding and sequestering essential trans-acting transcription factors .
	manualset3
95603	6	400703	13	NULL	NULL	NULL	NULL	trans-acting transcription factors 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the present study , we competed in-vitro transcription of circular template DNA with linear DNA fragments to identify promoter domains responsible for binding and sequestering essential trans-acting transcription factors .
	manualset3
98585	7	400703	13	NULL	NULL	0	NULL	sequestering 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we competed in-vitro transcription of circular template DNA with linear DNA fragments to identify promoter domains responsible for binding and sequestering essential trans-acting transcription factors .
	manualset3
95604	1	400704	13	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we evaluate our clinical experience of NPWT focusing on RV rupture and major bleeding complications and its potentially negative impact on 30-day mortality during an 11-year period .
	manualset3
95605	2	400704	13	NULL	NULL	0	NULL	clinical experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we evaluate our clinical experience of NPWT focusing on RV rupture and major bleeding complications and its potentially negative impact on 30-day mortality during an 11-year period .
	manualset3
95606	3	400704	13	NULL	NULL	0	NULL	NPWT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we evaluate our clinical experience of NPWT focusing on RV rupture and major bleeding complications and its potentially negative impact on 30-day mortality during an 11-year period .
	manualset3
95607	4	400704	13	NULL	NULL	0	NULL	focusing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we evaluate our clinical experience of NPWT focusing on RV rupture and major bleeding complications and its potentially negative impact on 30-day mortality during an 11-year period .
	manualset3
95608	5	400704	13	NULL	NULL	0	NULL	 RV rupture	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we evaluate our clinical experience of NPWT focusing on RV rupture and major bleeding complications and its potentially negative impact on 30-day mortality during an 11-year period .
	manualset3
95609	6	400704	13	NULL	NULL	0	NULL	major bleeding complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we evaluate our clinical experience of NPWT focusing on RV rupture and major bleeding complications and its potentially negative impact on 30-day mortality during an 11-year period .
	manualset3
95610	7	400704	13	NULL	NULL	0	NULL	negative impact	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we evaluate our clinical experience of NPWT focusing on RV rupture and major bleeding complications and its potentially negative impact on 30-day mortality during an 11-year period .
	manualset3
95611	8	400704	13	NULL	NULL	0	NULL	30-day 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we evaluate our clinical experience of NPWT focusing on RV rupture and major bleeding complications and its potentially negative impact on 30-day mortality during an 11-year period .
	manualset3
95612	9	400704	13	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we evaluate our clinical experience of NPWT focusing on RV rupture and major bleeding complications and its potentially negative impact on 30-day mortality during an 11-year period .
	manualset3
95613	10	400704	13	NULL	NULL	0	NULL	11-year period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we evaluate our clinical experience of NPWT focusing on RV rupture and major bleeding complications and its potentially negative impact on 30-day mortality during an 11-year period .
	manualset3
95614	1	400705	13	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we evaluated PCR coupled to restriction fragment length polymorphism to differentiate Taenia solium from Taenia saginata eggs present in fecal samples from naturally infected patients .
	manualset3
95615	2	400705	13	NULL	NULL	0	NULL	PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we evaluated PCR coupled to restriction fragment length polymorphism to differentiate Taenia solium from Taenia saginata eggs present in fecal samples from naturally infected patients .
	manualset3
95616	3	400705	13	NULL	NULL	0	NULL	restriction fragment length polymorphism	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we evaluated PCR coupled to restriction fragment length polymorphism to differentiate Taenia solium from Taenia saginata eggs present in fecal samples from naturally infected patients .
	manualset3
95617	4	400705	13	NULL	NULL	0	NULL	Taenia solium eggs 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we evaluated PCR coupled to restriction fragment length polymorphism to differentiate Taenia solium from Taenia saginata eggs present in fecal samples from naturally infected patients .
	manualset3
95618	5	400705	13	NULL	NULL	0	NULL	Taenia saginata eggs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we evaluated PCR coupled to restriction fragment length polymorphism to differentiate Taenia solium from Taenia saginata eggs present in fecal samples from naturally infected patients .
	manualset3
95619	6	400705	13	NULL	NULL	0	NULL	fecal samples	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we evaluated PCR coupled to restriction fragment length polymorphism to differentiate Taenia solium from Taenia saginata eggs present in fecal samples from naturally infected patients .
	manualset3
95620	7	400705	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we evaluated PCR coupled to restriction fragment length polymorphism to differentiate Taenia solium from Taenia saginata eggs present in fecal samples from naturally infected patients .
	manualset3
95621	1	400706	13	NULL	NULL	0	NULL	present study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we exposed rat cortical neurons to hypoxia ( 1 % O2 ) and examined the effects of three major inhibitory neurotransmitters ( GABA , glycine and taurine ) on the hypoxic neurons at different neuronal ages ( days in vitro ( DIV ) 4-20 ) .
	manualset3
95622	2	400706	13	NULL	NULL	0	NULL	 rat cortical neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we exposed rat cortical neurons to hypoxia ( 1 % O2 ) and examined the effects of three major inhibitory neurotransmitters ( GABA , glycine and taurine ) on the hypoxic neurons at different neuronal ages ( days in vitro ( DIV ) 4-20 ) .
	manualset3
95623	3	400706	13	NULL	NULL	0	NULL	hypoxia	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we exposed rat cortical neurons to hypoxia ( 1 % O2 ) and examined the effects of three major inhibitory neurotransmitters ( GABA , glycine and taurine ) on the hypoxic neurons at different neuronal ages ( days in vitro ( DIV ) 4-20 ) .
	manualset3
95624	4	400706	13	NULL	NULL	0	NULL	1 % O2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we exposed rat cortical neurons to hypoxia ( 1 % O2 ) and examined the effects of three major inhibitory neurotransmitters ( GABA , glycine and taurine ) on the hypoxic neurons at different neuronal ages ( days in vitro ( DIV ) 4-20 ) .
	manualset3
95625	5	400706	13	NULL	NULL	0	NULL	effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we exposed rat cortical neurons to hypoxia ( 1 % O2 ) and examined the effects of three major inhibitory neurotransmitters ( GABA , glycine and taurine ) on the hypoxic neurons at different neuronal ages ( days in vitro ( DIV ) 4-20 ) .
	manualset3
95626	6	400706	13	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we exposed rat cortical neurons to hypoxia ( 1 % O2 ) and examined the effects of three major inhibitory neurotransmitters ( GABA , glycine and taurine ) on the hypoxic neurons at different neuronal ages ( days in vitro ( DIV ) 4-20 ) .
	manualset3
95627	7	400706	13	NULL	NULL	0	NULL	major inhibitory neurotransmitters	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we exposed rat cortical neurons to hypoxia ( 1 % O2 ) and examined the effects of three major inhibitory neurotransmitters ( GABA , glycine and taurine ) on the hypoxic neurons at different neuronal ages ( days in vitro ( DIV ) 4-20 ) .
	manualset3
95628	8	400706	13	NULL	NULL	NULL	NULL	GABA	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the present study , we exposed rat cortical neurons to hypoxia ( 1 % O2 ) and examined the effects of three major inhibitory neurotransmitters ( GABA , glycine and taurine ) on the hypoxic neurons at different neuronal ages ( days in vitro ( DIV ) 4-20 ) .
	manualset3
95629	9	400706	13	NULL	NULL	NULL	NULL	glycine	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the present study , we exposed rat cortical neurons to hypoxia ( 1 % O2 ) and examined the effects of three major inhibitory neurotransmitters ( GABA , glycine and taurine ) on the hypoxic neurons at different neuronal ages ( days in vitro ( DIV ) 4-20 ) .
	manualset3
95630	10	400706	13	NULL	NULL	0	NULL	taurine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we exposed rat cortical neurons to hypoxia ( 1 % O2 ) and examined the effects of three major inhibitory neurotransmitters ( GABA , glycine and taurine ) on the hypoxic neurons at different neuronal ages ( days in vitro ( DIV ) 4-20 ) .
	manualset3
95631	11	400706	13	NULL	NULL	0	NULL	hypoxic neurons 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we exposed rat cortical neurons to hypoxia ( 1 % O2 ) and examined the effects of three major inhibitory neurotransmitters ( GABA , glycine and taurine ) on the hypoxic neurons at different neuronal ages ( days in vitro ( DIV ) 4-20 ) .
	manualset3
95632	12	400706	13	NULL	NULL	0	NULL	neuronal ages	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we exposed rat cortical neurons to hypoxia ( 1 % O2 ) and examined the effects of three major inhibitory neurotransmitters ( GABA , glycine and taurine ) on the hypoxic neurons at different neuronal ages ( days in vitro ( DIV ) 4-20 ) .
	manualset3
95633	13	400706	13	NULL	NULL	0	NULL	days in vitro ( DIV ) 4-20	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we exposed rat cortical neurons to hypoxia ( 1 % O2 ) and examined the effects of three major inhibitory neurotransmitters ( GABA , glycine and taurine ) on the hypoxic neurons at different neuronal ages ( days in vitro ( DIV ) 4-20 ) .
	manualset3
95634	1	400707	13	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we have assessed the level of gene expression of some cytokines in the NTS of SHR compared to WKY .
	manualset3
95635	2	400707	13	NULL	NULL	0	NULL	level of gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we have assessed the level of gene expression of some cytokines in the NTS of SHR compared to WKY .
	manualset3
95636	3	400707	13	NULL	NULL	0	NULL	cytokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we have assessed the level of gene expression of some cytokines in the NTS of SHR compared to WKY .
	manualset3
95637	4	400707	13	NULL	NULL	0	NULL	NTS	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we have assessed the level of gene expression of some cytokines in the NTS of SHR compared to WKY .
	manualset3
95638	5	400707	13	NULL	NULL	0	NULL	SHR	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we have assessed the level of gene expression of some cytokines in the NTS of SHR compared to WKY .
	manualset3
95639	6	400707	13	NULL	NULL	0	NULL	WKY	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we have assessed the level of gene expression of some cytokines in the NTS of SHR compared to WKY .
	manualset3
95640	1	400708	13	NULL	NULL	0	NULL	present study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we have investigated the function of the receptor protein tyrosine phosphatase alpha ( RPTP alpha ) in the neuronal differentiation of E14-embryonic stem ( E14-ES ) cells .
	manualset3
95641	2	400708	13	NULL	NULL	0	NULL	function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we have investigated the function of the receptor protein tyrosine phosphatase alpha ( RPTP alpha ) in the neuronal differentiation of E14-embryonic stem ( E14-ES ) cells .
	manualset3
95642	3	400708	13	NULL	NULL	0	NULL	receptor protein tyrosine phosphatase alpha ( RPTP alpha )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we have investigated the function of the receptor protein tyrosine phosphatase alpha ( RPTP alpha ) in the neuronal differentiation of E14-embryonic stem ( E14-ES ) cells .
	manualset3
95643	4	400708	13	NULL	NULL	0	NULL	neuronal differentiation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we have investigated the function of the receptor protein tyrosine phosphatase alpha ( RPTP alpha ) in the neuronal differentiation of E14-embryonic stem ( E14-ES ) cells .
	manualset3
95644	5	400708	13	NULL	NULL	0	NULL	E14-embryonic stem ( E14-ES ) cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we have investigated the function of the receptor protein tyrosine phosphatase alpha ( RPTP alpha ) in the neuronal differentiation of E14-embryonic stem ( E14-ES ) cells .
	manualset3
95645	1	400709	13	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we have observed c-Jun induction in cells sensitive to ionizing radiation during the whole process of radiation-induced cell death , and that this expression is accompanied by modifications in the composition of AP-1 complexes : c-Jun/AP -1 activity is highly increased whereas Jun D/AP -1 is slightly decreased .
	manualset3
95646	2	400709	13	NULL	NULL	0	NULL	c-Jun induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we have observed c-Jun induction in cells sensitive to ionizing radiation during the whole process of radiation-induced cell death , and that this expression is accompanied by modifications in the composition of AP-1 complexes : c-Jun/AP -1 activity is highly increased whereas Jun D/AP -1 is slightly decreased .
	manualset3
95647	3	400709	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we have observed c-Jun induction in cells sensitive to ionizing radiation during the whole process of radiation-induced cell death , and that this expression is accompanied by modifications in the composition of AP-1 complexes : c-Jun/AP -1 activity is highly increased whereas Jun D/AP -1 is slightly decreased .
	manualset3
95648	4	400709	13	NULL	NULL	NULL	NULL	radiation	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the present study , we have observed c-Jun induction in cells sensitive to ionizing radiation during the whole process of radiation-induced cell death , and that this expression is accompanied by modifications in the composition of AP-1 complexes : c-Jun/AP -1 activity is highly increased whereas Jun D/AP -1 is slightly decreased .
	manualset3
95649	5	400709	13	NULL	NULL	0	NULL	process of radiation-induced cell death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we have observed c-Jun induction in cells sensitive to ionizing radiation during the whole process of radiation-induced cell death , and that this expression is accompanied by modifications in the composition of AP-1 complexes : c-Jun/AP -1 activity is highly increased whereas Jun D/AP -1 is slightly decreased .
	manualset3
95650	6	400709	13	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we have observed c-Jun induction in cells sensitive to ionizing radiation during the whole process of radiation-induced cell death , and that this expression is accompanied by modifications in the composition of AP-1 complexes : c-Jun/AP -1 activity is highly increased whereas Jun D/AP -1 is slightly decreased .
	manualset3
95651	7	400709	13	NULL	NULL	0	NULL	modifications	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we have observed c-Jun induction in cells sensitive to ionizing radiation during the whole process of radiation-induced cell death , and that this expression is accompanied by modifications in the composition of AP-1 complexes : c-Jun/AP -1 activity is highly increased whereas Jun D/AP -1 is slightly decreased .
	manualset3
95652	8	400709	13	NULL	NULL	0	NULL	composition of AP-1 complexes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we have observed c-Jun induction in cells sensitive to ionizing radiation during the whole process of radiation-induced cell death , and that this expression is accompanied by modifications in the composition of AP-1 complexes : c-Jun/AP -1 activity is highly increased whereas Jun D/AP -1 is slightly decreased .
	manualset3
95653	9	400709	13	NULL	NULL	0	NULL	c-Jun/AP -1 activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we have observed c-Jun induction in cells sensitive to ionizing radiation during the whole process of radiation-induced cell death , and that this expression is accompanied by modifications in the composition of AP-1 complexes : c-Jun/AP -1 activity is highly increased whereas Jun D/AP -1 is slightly decreased .
	manualset3
95654	10	400709	13	NULL	NULL	0	NULL	Jun D/AP -1 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we have observed c-Jun induction in cells sensitive to ionizing radiation during the whole process of radiation-induced cell death , and that this expression is accompanied by modifications in the composition of AP-1 complexes : c-Jun/AP -1 activity is highly increased whereas Jun D/AP -1 is slightly decreased .
	manualset3
95655	1	400710	13	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated the concentration of CS , heparan sulfate ( HS ) and hyaluronic acid ( HA ) in the hippocampus and temporal neocortex as well as RPTP zeta/beta expression in the hippocampus of patients with MTLE .
	manualset3
95656	2	400710	13	NULL	NULL	0	NULL	concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated the concentration of CS , heparan sulfate ( HS ) and hyaluronic acid ( HA ) in the hippocampus and temporal neocortex as well as RPTP zeta/beta expression in the hippocampus of patients with MTLE .
	manualset3
95657	3	400710	13	NULL	NULL	0	NULL	CS 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated the concentration of CS , heparan sulfate ( HS ) and hyaluronic acid ( HA ) in the hippocampus and temporal neocortex as well as RPTP zeta/beta expression in the hippocampus of patients with MTLE .
	manualset3
95658	4	400710	13	NULL	NULL	0	NULL	heparan sulfate ( HS )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated the concentration of CS , heparan sulfate ( HS ) and hyaluronic acid ( HA ) in the hippocampus and temporal neocortex as well as RPTP zeta/beta expression in the hippocampus of patients with MTLE .
	manualset3
95659	5	400710	13	NULL	NULL	0	NULL	hyaluronic acid ( HA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated the concentration of CS , heparan sulfate ( HS ) and hyaluronic acid ( HA ) in the hippocampus and temporal neocortex as well as RPTP zeta/beta expression in the hippocampus of patients with MTLE .
	manualset3
95660	6	400710	13	NULL	NULL	0	NULL	hippocampus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated the concentration of CS , heparan sulfate ( HS ) and hyaluronic acid ( HA ) in the hippocampus and temporal neocortex as well as RPTP zeta/beta expression in the hippocampus of patients with MTLE .
	manualset3
95661	7	400710	13	NULL	NULL	0	NULL	temporal neocortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated the concentration of CS , heparan sulfate ( HS ) and hyaluronic acid ( HA ) in the hippocampus and temporal neocortex as well as RPTP zeta/beta expression in the hippocampus of patients with MTLE .
	manualset3
95662	8	400710	13	NULL	NULL	0	NULL	RPTP zeta/beta expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated the concentration of CS , heparan sulfate ( HS ) and hyaluronic acid ( HA ) in the hippocampus and temporal neocortex as well as RPTP zeta/beta expression in the hippocampus of patients with MTLE .
	manualset3
95663	9	400710	13	NULL	NULL	0	NULL	hippocampus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated the concentration of CS , heparan sulfate ( HS ) and hyaluronic acid ( HA ) in the hippocampus and temporal neocortex as well as RPTP zeta/beta expression in the hippocampus of patients with MTLE .
	manualset3
95664	10	400710	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated the concentration of CS , heparan sulfate ( HS ) and hyaluronic acid ( HA ) in the hippocampus and temporal neocortex as well as RPTP zeta/beta expression in the hippocampus of patients with MTLE .
	manualset3
95665	11	400710	13	NULL	NULL	0	NULL	MTLE	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated the concentration of CS , heparan sulfate ( HS ) and hyaluronic acid ( HA ) in the hippocampus and temporal neocortex as well as RPTP zeta/beta expression in the hippocampus of patients with MTLE .
	manualset3
95666	1	400711	13	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated the effect of the anti-inflammatory cytokine transforming growth factor-beta ( TGF-beta ) on TLR2 expression in primary-cultured murine hepatocytes .
	manualset3
95667	2	400711	13	NULL	NULL	0	NULL	effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated the effect of the anti-inflammatory cytokine transforming growth factor-beta ( TGF-beta ) on TLR2 expression in primary-cultured murine hepatocytes .
	manualset3
95668	3	400711	13	NULL	NULL	0	NULL	anti-inflammatory cytokine transforming growth factor-beta ( TGF-beta )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated the effect of the anti-inflammatory cytokine transforming growth factor-beta ( TGF-beta ) on TLR2 expression in primary-cultured murine hepatocytes .
	manualset3
95669	4	400711	13	NULL	NULL	0	NULL	TLR2 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated the effect of the anti-inflammatory cytokine transforming growth factor-beta ( TGF-beta ) on TLR2 expression in primary-cultured murine hepatocytes .
	manualset3
95670	5	400711	13	NULL	NULL	0	NULL	primary-cultured murine hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated the effect of the anti-inflammatory cytokine transforming growth factor-beta ( TGF-beta ) on TLR2 expression in primary-cultured murine hepatocytes .
	manualset3
95671	1	400712	13	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated the effects of various Ca2 + blockers on the release of acetylcholine ( ACh ) induced by nicotine , electrical field stimulation ( EFS ) and high-K + .
	manualset3
95672	2	400712	13	NULL	NULL	0	NULL	effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated the effects of various Ca2 + blockers on the release of acetylcholine ( ACh ) induced by nicotine , electrical field stimulation ( EFS ) and high-K + .
	manualset3
95673	3	400712	13	NULL	NULL	0	NULL	 Ca2 + blockers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated the effects of various Ca2 + blockers on the release of acetylcholine ( ACh ) induced by nicotine , electrical field stimulation ( EFS ) and high-K + .
	manualset3
95674	4	400712	13	NULL	NULL	0	NULL	release of acetylcholine ( ACh ) 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated the effects of various Ca2 + blockers on the release of acetylcholine ( ACh ) induced by nicotine , electrical field stimulation ( EFS ) and high-K + .
	manualset3
95675	5	400712	13	NULL	NULL	0	NULL	nicotine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated the effects of various Ca2 + blockers on the release of acetylcholine ( ACh ) induced by nicotine , electrical field stimulation ( EFS ) and high-K + .
	manualset3
95676	6	400712	13	NULL	NULL	0	NULL	electrical field stimulation ( EFS )	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated the effects of various Ca2 + blockers on the release of acetylcholine ( ACh ) induced by nicotine , electrical field stimulation ( EFS ) and high-K + .
	manualset3
95677	7	400712	13	NULL	NULL	0	NULL	high-K +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated the effects of various Ca2 + blockers on the release of acetylcholine ( ACh ) induced by nicotine , electrical field stimulation ( EFS ) and high-K + .
	manualset3
95678	1	400713	13	NULL	NULL	0	NULL	 present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated the relationship between Fbw7 and PKC .
	manualset3
95679	2	400713	13	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated the relationship between Fbw7 and PKC .
	manualset3
95680	3	400713	13	NULL	NULL	0	NULL	 Fbw7	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated the relationship between Fbw7 and PKC .
	manualset3
95681	4	400713	13	NULL	NULL	0	NULL	PKC	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated the relationship between Fbw7 and PKC .
	manualset3
95682	1	400714	13	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated whether H3-receptors modulate nonexocytotic norepinephrine release during protracted myocardial ischemia .
	manualset3
95683	2	400714	13	NULL	NULL	0	NULL	H3-receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated whether H3-receptors modulate nonexocytotic norepinephrine release during protracted myocardial ischemia .
	manualset3
95684	3	400714	13	NULL	NULL	0	NULL	nonexocytotic norepinephrine release 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated whether H3-receptors modulate nonexocytotic norepinephrine release during protracted myocardial ischemia .
	manualset3
95685	4	400714	13	NULL	NULL	0	NULL	protracted myocardial ischemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated whether H3-receptors modulate nonexocytotic norepinephrine release during protracted myocardial ischemia .
	manualset3
95686	1	400715	13	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated whether PGE2 regulated interleukin ( IL ) -1 beta-induced matrix metalloproteinase ( MMP ) -3 production in human gingival fibroblasts ( HGF ) derived from periodontally healthy subjects and diseased patients .
	manualset3
95687	2	400715	13	NULL	NULL	0	NULL	 PGE2 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated whether PGE2 regulated interleukin ( IL ) -1 beta-induced matrix metalloproteinase ( MMP ) -3 production in human gingival fibroblasts ( HGF ) derived from periodontally healthy subjects and diseased patients .
	manualset3
95688	3	400715	13	NULL	NULL	0	NULL	 interleukin ( IL ) -1 beta-induced matrix metalloproteinase ( MMP ) -3 production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated whether PGE2 regulated interleukin ( IL ) -1 beta-induced matrix metalloproteinase ( MMP ) -3 production in human gingival fibroblasts ( HGF ) derived from periodontally healthy subjects and diseased patients .
	manualset3
95689	4	400715	13	NULL	NULL	0	NULL	human gingival fibroblasts ( HGF )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated whether PGE2 regulated interleukin ( IL ) -1 beta-induced matrix metalloproteinase ( MMP ) -3 production in human gingival fibroblasts ( HGF ) derived from periodontally healthy subjects and diseased patients .
	manualset3
95690	5	400715	13	NULL	NULL	0	NULL	healthy subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated whether PGE2 regulated interleukin ( IL ) -1 beta-induced matrix metalloproteinase ( MMP ) -3 production in human gingival fibroblasts ( HGF ) derived from periodontally healthy subjects and diseased patients .
	manualset3
95691	6	400715	13	NULL	NULL	0	NULL	diseased patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we investigated whether PGE2 regulated interleukin ( IL ) -1 beta-induced matrix metalloproteinase ( MMP ) -3 production in human gingival fibroblasts ( HGF ) derived from periodontally healthy subjects and diseased patients .
	manualset3
95692	1	400716	13	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we report the case of a patient who presented with neonatal blistering and late-onset muscular dystrophy with nail and tooth abnormalities , as well as severe mucocutaneous involvement including laryngeal webs and urethral strictures , features not previously reported in this syndrome .
	manualset3
95693	2	400716	13	NULL	NULL	0	NULL	case of a patient	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we report the case of a patient who presented with neonatal blistering and late-onset muscular dystrophy with nail and tooth abnormalities , as well as severe mucocutaneous involvement including laryngeal webs and urethral strictures , features not previously reported in this syndrome .
	manualset3
95694	3	400716	13	NULL	NULL	0	NULL	neonatal blistering	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we report the case of a patient who presented with neonatal blistering and late-onset muscular dystrophy with nail and tooth abnormalities , as well as severe mucocutaneous involvement including laryngeal webs and urethral strictures , features not previously reported in this syndrome .
	manualset3
95695	4	400716	13	NULL	NULL	0	NULL	late-onset muscular dystrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we report the case of a patient who presented with neonatal blistering and late-onset muscular dystrophy with nail and tooth abnormalities , as well as severe mucocutaneous involvement including laryngeal webs and urethral strictures , features not previously reported in this syndrome .
	manualset3
95696	5	400716	13	NULL	NULL	0	NULL	nail abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we report the case of a patient who presented with neonatal blistering and late-onset muscular dystrophy with nail and tooth abnormalities , as well as severe mucocutaneous involvement including laryngeal webs and urethral strictures , features not previously reported in this syndrome .
	manualset3
95697	6	400716	13	NULL	NULL	0	NULL	tooth abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we report the case of a patient who presented with neonatal blistering and late-onset muscular dystrophy with nail and tooth abnormalities , as well as severe mucocutaneous involvement including laryngeal webs and urethral strictures , features not previously reported in this syndrome .
	manualset3
95698	7	400716	13	NULL	NULL	0	NULL	severe mucocutaneous involvement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we report the case of a patient who presented with neonatal blistering and late-onset muscular dystrophy with nail and tooth abnormalities , as well as severe mucocutaneous involvement including laryngeal webs and urethral strictures , features not previously reported in this syndrome .
	manualset3
95699	8	400716	13	NULL	NULL	0	NULL	laryngeal webs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we report the case of a patient who presented with neonatal blistering and late-onset muscular dystrophy with nail and tooth abnormalities , as well as severe mucocutaneous involvement including laryngeal webs and urethral strictures , features not previously reported in this syndrome .
	manualset3
95700	9	400716	13	NULL	NULL	0	NULL	urethral strictures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we report the case of a patient who presented with neonatal blistering and late-onset muscular dystrophy with nail and tooth abnormalities , as well as severe mucocutaneous involvement including laryngeal webs and urethral strictures , features not previously reported in this syndrome .
	manualset3
95701	10	400716	13	NULL	NULL	0	NULL	features	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we report the case of a patient who presented with neonatal blistering and late-onset muscular dystrophy with nail and tooth abnormalities , as well as severe mucocutaneous involvement including laryngeal webs and urethral strictures , features not previously reported in this syndrome .
	manualset3
95702	11	400716	13	NULL	NULL	0	NULL	syndrome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we report the case of a patient who presented with neonatal blistering and late-onset muscular dystrophy with nail and tooth abnormalities , as well as severe mucocutaneous involvement including laryngeal webs and urethral strictures , features not previously reported in this syndrome .
	manualset3
95703	1	400717	13	NULL	NULL	0	NULL	 present study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we show that in addition to acutely inhibiting ERAD ( ER-associated degradation ) , ESI causes production of mislocalized polypeptides that are ubiquitinated and degraded .
	manualset3
95704	2	400717	13	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we show that in addition to acutely inhibiting ERAD ( ER-associated degradation ) , ESI causes production of mislocalized polypeptides that are ubiquitinated and degraded .
	manualset3
95705	3	400717	13	NULL	NULL	0	NULL	ERAD ( ER-associated degradation ) 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we show that in addition to acutely inhibiting ERAD ( ER-associated degradation ) , ESI causes production of mislocalized polypeptides that are ubiquitinated and degraded .
	manualset3
95706	4	400717	13	NULL	NULL	0	NULL	ESI 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we show that in addition to acutely inhibiting ERAD ( ER-associated degradation ) , ESI causes production of mislocalized polypeptides that are ubiquitinated and degraded .
	manualset3
95708	6	400717	13	NULL	NULL	NULL	NULL	production 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the present study , we show that in addition to acutely inhibiting ERAD ( ER-associated degradation ) , ESI causes production of mislocalized polypeptides that are ubiquitinated and degraded .
	manualset3
95709	7	400717	13	NULL	NULL	0	NULL	polypeptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we show that in addition to acutely inhibiting ERAD ( ER-associated degradation ) , ESI causes production of mislocalized polypeptides that are ubiquitinated and degraded .
	manualset3
95710	1	400718	13	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we tested if intact ghrelin signaling is required for FEO function by studying food anticipatory activity ( FAA ) in preproghrelin knockout ( KO ) and wild-type ( WT ) mice .
	manualset3
95711	2	400718	13	NULL	NULL	0	NULL	ghrelin signaling 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we tested if intact ghrelin signaling is required for FEO function by studying food anticipatory activity ( FAA ) in preproghrelin knockout ( KO ) and wild-type ( WT ) mice .
	manualset3
95712	3	400718	13	NULL	NULL	0	NULL	FEO function 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we tested if intact ghrelin signaling is required for FEO function by studying food anticipatory activity ( FAA ) in preproghrelin knockout ( KO ) and wild-type ( WT ) mice .
	manualset3
95713	4	400718	13	NULL	NULL	0	NULL	 food anticipatory activity ( FAA )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we tested if intact ghrelin signaling is required for FEO function by studying food anticipatory activity ( FAA ) in preproghrelin knockout ( KO ) and wild-type ( WT ) mice .
	manualset3
95714	5	400718	13	NULL	NULL	0	NULL	preproghrelin knockout ( KO ) mice  	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we tested if intact ghrelin signaling is required for FEO function by studying food anticipatory activity ( FAA ) in preproghrelin knockout ( KO ) and wild-type ( WT ) mice .
	manualset3
95715	6	400718	13	NULL	NULL	0	NULL	wild-type ( WT ) mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we tested if intact ghrelin signaling is required for FEO function by studying food anticipatory activity ( FAA ) in preproghrelin knockout ( KO ) and wild-type ( WT ) mice .
	manualset3
95716	1	400719	13	NULL	NULL	0	NULL	104 women	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	104 out of 142 women living in the community were enrolled , and semistructured questionnaires containing questions concerning demographic , sociocultural , obstetrical , gynecological information and diagnosis were administered .
	manualset3
95717	2	400719	13	NULL	NULL	0	NULL	142 women	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	104 out of 142 women living in the community were enrolled , and semistructured questionnaires containing questions concerning demographic , sociocultural , obstetrical , gynecological information and diagnosis were administered .
	manualset3
95718	3	400719	13	NULL	NULL	0	NULL	community	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	104 out of 142 women living in the community were enrolled , and semistructured questionnaires containing questions concerning demographic , sociocultural , obstetrical , gynecological information and diagnosis were administered .
	manualset3
95719	4	400719	13	NULL	NULL	NULL	NULL	questionnaires	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	104 out of 142 women living in the community were enrolled , and semistructured questionnaires containing questions concerning demographic , sociocultural , obstetrical , gynecological information and diagnosis were administered .
	manualset3
95720	5	400719	13	NULL	NULL	0	NULL	questions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	104 out of 142 women living in the community were enrolled , and semistructured questionnaires containing questions concerning demographic , sociocultural , obstetrical , gynecological information and diagnosis were administered .
	manualset3
95721	6	400719	13	NULL	NULL	0	NULL	demographic information 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	104 out of 142 women living in the community were enrolled , and semistructured questionnaires containing questions concerning demographic , sociocultural , obstetrical , gynecological information and diagnosis were administered .
	manualset3
95722	7	400719	13	NULL	NULL	0	NULL	sociocultural information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	104 out of 142 women living in the community were enrolled , and semistructured questionnaires containing questions concerning demographic , sociocultural , obstetrical , gynecological information and diagnosis were administered .
	manualset3
95723	8	400719	13	NULL	NULL	0	NULL	obstetrical information 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	104 out of 142 women living in the community were enrolled , and semistructured questionnaires containing questions concerning demographic , sociocultural , obstetrical , gynecological information and diagnosis were administered .
	manualset3
95724	9	400719	13	NULL	NULL	0	NULL	gynecological information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	104 out of 142 women living in the community were enrolled , and semistructured questionnaires containing questions concerning demographic , sociocultural , obstetrical , gynecological information and diagnosis were administered .
	manualset3
95725	10	400719	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	104 out of 142 women living in the community were enrolled , and semistructured questionnaires containing questions concerning demographic , sociocultural , obstetrical , gynecological information and diagnosis were administered .
	manualset3
95726	1	400720	13	NULL	NULL	0	NULL	 present study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we tested various functions of murine peritoneal macrophages that were isolated and stimulated with LPS after AFB1 ( 400 microg/5 ml/kg ) was administered every other day for 2 weeks .
	manualset3
95727	2	400720	13	NULL	NULL	0	NULL	various functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we tested various functions of murine peritoneal macrophages that were isolated and stimulated with LPS after AFB1 ( 400 microg/5 ml/kg ) was administered every other day for 2 weeks .
	manualset3
95728	3	400720	13	NULL	NULL	0	NULL	murine peritoneal macrophages 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we tested various functions of murine peritoneal macrophages that were isolated and stimulated with LPS after AFB1 ( 400 microg/5 ml/kg ) was administered every other day for 2 weeks .
	manualset3
95729	4	400720	13	NULL	NULL	0	NULL	LPS	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we tested various functions of murine peritoneal macrophages that were isolated and stimulated with LPS after AFB1 ( 400 microg/5 ml/kg ) was administered every other day for 2 weeks .
	manualset3
95730	5	400720	13	NULL	NULL	0	NULL	AFB1	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we tested various functions of murine peritoneal macrophages that were isolated and stimulated with LPS after AFB1 ( 400 microg/5 ml/kg ) was administered every other day for 2 weeks .
	manualset3
95731	6	400720	13	NULL	NULL	0	NULL	400 microg/5 ml/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we tested various functions of murine peritoneal macrophages that were isolated and stimulated with LPS after AFB1 ( 400 microg/5 ml/kg ) was administered every other day for 2 weeks .
	manualset3
95732	7	400720	13	NULL	NULL	0	NULL	2 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study , we tested various functions of murine peritoneal macrophages that were isolated and stimulated with LPS after AFB1 ( 400 microg/5 ml/kg ) was administered every other day for 2 weeks .
	manualset3
95733	1	400721	13	NULL	NULL	0	NULL	 present study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study an axenic amastigote culture was used to study the in vitro responses of Leishmania donovani to SbV .
	manualset3
95734	2	400721	13	NULL	NULL	0	NULL	axenic amastigote culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study an axenic amastigote culture was used to study the in vitro responses of Leishmania donovani to SbV .
	manualset3
95735	3	400721	13	NULL	NULL	0	NULL	in vitro responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study an axenic amastigote culture was used to study the in vitro responses of Leishmania donovani to SbV .
	manualset3
95736	4	400721	13	NULL	NULL	0	NULL	Leishmania donovani	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study an axenic amastigote culture was used to study the in vitro responses of Leishmania donovani to SbV .
	manualset3
95737	5	400721	13	NULL	NULL	0	NULL	SbV	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study an axenic amastigote culture was used to study the in vitro responses of Leishmania donovani to SbV .
	manualset3
95738	1	400722	13	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study effects of nitroglycerin ( NG ) and 4-aminopyridine ( 4-AP ) on ( Ca + + ) ; and contraction were studied .
	manualset3
95739	2	400722	13	NULL	NULL	0	NULL	effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study effects of nitroglycerin ( NG ) and 4-aminopyridine ( 4-AP ) on ( Ca + + ) ; and contraction were studied .
	manualset3
95740	3	400722	13	NULL	NULL	0	NULL	nitroglycerin ( NG ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study effects of nitroglycerin ( NG ) and 4-aminopyridine ( 4-AP ) on ( Ca + + ) ; and contraction were studied .
	manualset3
95741	4	400722	13	NULL	NULL	0	NULL	 4-aminopyridine ( 4-AP ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study effects of nitroglycerin ( NG ) and 4-aminopyridine ( 4-AP ) on ( Ca + + ) ; and contraction were studied .
	manualset3
95742	5	400722	13	NULL	NULL	0	NULL	Ca + +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study effects of nitroglycerin ( NG ) and 4-aminopyridine ( 4-AP ) on ( Ca + + ) ; and contraction were studied .
	manualset3
95743	6	400722	13	NULL	NULL	0	NULL	contraction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study effects of nitroglycerin ( NG ) and 4-aminopyridine ( 4-AP ) on ( Ca + + ) ; and contraction were studied .
	manualset3
95744	1	400723	13	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study the clearly defined anatomical region of the tongue was analyzed for potentially specific patterns of chromosomal alterations .
	manualset3
95745	2	400723	13	NULL	NULL	0	NULL	anatomical region of the tongue 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study the clearly defined anatomical region of the tongue was analyzed for potentially specific patterns of chromosomal alterations .
	manualset3
95746	3	400723	13	NULL	NULL	0	NULL	specific patterns of chromosomal alterations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study the clearly defined anatomical region of the tongue was analyzed for potentially specific patterns of chromosomal alterations .
	manualset3
95747	1	400724	13	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study the effects of intraduodenal ( i.d. ) fat ( endogenous CCK ) and of CCK infusion on satiety were studied during normo-and hyperglycemic conditions .
	manualset3
95748	2	400724	13	NULL	NULL	0	NULL	effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study the effects of intraduodenal ( i.d. ) fat ( endogenous CCK ) and of CCK infusion on satiety were studied during normo-and hyperglycemic conditions .
	manualset3
95749	3	400724	13	NULL	NULL	0	NULL	intraduodenal ( i.d. ) fat	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study the effects of intraduodenal ( i.d. ) fat ( endogenous CCK ) and of CCK infusion on satiety were studied during normo-and hyperglycemic conditions .
	manualset3
95750	4	400724	13	NULL	NULL	0	NULL	endogenous CCK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study the effects of intraduodenal ( i.d. ) fat ( endogenous CCK ) and of CCK infusion on satiety were studied during normo-and hyperglycemic conditions .
	manualset3
95751	5	400724	13	NULL	NULL	0	NULL	CCK infusion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study the effects of intraduodenal ( i.d. ) fat ( endogenous CCK ) and of CCK infusion on satiety were studied during normo-and hyperglycemic conditions .
	manualset3
95752	6	400724	13	NULL	NULL	0	NULL	satiety	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study the effects of intraduodenal ( i.d. ) fat ( endogenous CCK ) and of CCK infusion on satiety were studied during normo-and hyperglycemic conditions .
	manualset3
95753	7	400724	13	NULL	NULL	NULL	NULL	normoglycemic-conditions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the present study the effects of intraduodenal ( i.d. ) fat ( endogenous CCK ) and of CCK infusion on satiety were studied during normo-and hyperglycemic conditions .
	manualset3
95754	8	400724	13	NULL	NULL	0	NULL	hyperglycemic conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study the effects of intraduodenal ( i.d. ) fat ( endogenous CCK ) and of CCK infusion on satiety were studied during normo-and hyperglycemic conditions .
	manualset3
95755	1	400725	13	NULL	NULL	0	NULL	present study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study therapists ' adherence and perceptions of the manual are studied .
	manualset3
95756	2	400725	13	NULL	NULL	0	NULL	therapists '	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study therapists ' adherence and perceptions of the manual are studied .
	manualset3
95757	3	400725	13	NULL	NULL	0	NULL	adherence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study therapists ' adherence and perceptions of the manual are studied .
	manualset3
95758	4	400725	13	NULL	NULL	0	NULL	perceptions	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study therapists ' adherence and perceptions of the manual are studied .
	manualset3
95759	5	400725	13	NULL	NULL	0	NULL	manual 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study therapists ' adherence and perceptions of the manual are studied .
	manualset3
95760	1	400726	13	NULL	NULL	0	NULL	present study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study we determined the effect of chronic administration of homocysteine on Na + , K + - ATPase activity in synaptic membranes from parietal , prefrontal and cingulate cortex of young rats .
	manualset3
95761	2	400726	13	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study we determined the effect of chronic administration of homocysteine on Na + , K + - ATPase activity in synaptic membranes from parietal , prefrontal and cingulate cortex of young rats .
	manualset3
95762	3	400726	13	NULL	NULL	0	NULL	chronic administration	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study we determined the effect of chronic administration of homocysteine on Na + , K + - ATPase activity in synaptic membranes from parietal , prefrontal and cingulate cortex of young rats .
	manualset3
95763	4	400726	13	NULL	NULL	0	NULL	homocysteine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study we determined the effect of chronic administration of homocysteine on Na + , K + - ATPase activity in synaptic membranes from parietal , prefrontal and cingulate cortex of young rats .
	manualset3
95764	5	400726	13	NULL	NULL	0	NULL	 Na +- ATPase activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study we determined the effect of chronic administration of homocysteine on Na + , K + - ATPase activity in synaptic membranes from parietal , prefrontal and cingulate cortex of young rats .
	manualset3
95765	6	400726	13	NULL	NULL	0	NULL	 K + - ATPase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study we determined the effect of chronic administration of homocysteine on Na + , K + - ATPase activity in synaptic membranes from parietal , prefrontal and cingulate cortex of young rats .
	manualset3
95766	7	400726	13	NULL	NULL	0	NULL	synaptic membranes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study we determined the effect of chronic administration of homocysteine on Na + , K + - ATPase activity in synaptic membranes from parietal , prefrontal and cingulate cortex of young rats .
	manualset3
95767	8	400726	13	NULL	NULL	0	NULL	parietal cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study we determined the effect of chronic administration of homocysteine on Na + , K + - ATPase activity in synaptic membranes from parietal , prefrontal and cingulate cortex of young rats .
	manualset3
95768	9	400726	13	NULL	NULL	0	NULL	prefrontal cortex 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study we determined the effect of chronic administration of homocysteine on Na + , K + - ATPase activity in synaptic membranes from parietal , prefrontal and cingulate cortex of young rats .
	manualset3
95769	10	400726	13	NULL	NULL	0	NULL	cingulate cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study we determined the effect of chronic administration of homocysteine on Na + , K + - ATPase activity in synaptic membranes from parietal , prefrontal and cingulate cortex of young rats .
	manualset3
95770	11	400726	13	NULL	NULL	0	NULL	young rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study we determined the effect of chronic administration of homocysteine on Na + , K + - ATPase activity in synaptic membranes from parietal , prefrontal and cingulate cortex of young rats .
	manualset3
95771	1	400727	13	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study we estimated serum GlcNAc-phosphotransferase in 50 adults suffering from leukemia and myelodysplastic syndrome .
	manualset3
95772	2	400727	13	NULL	NULL	NULL	NULL	serum GlcNAc-phosphotransferase 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the present study we estimated serum GlcNAc-phosphotransferase in 50 adults suffering from leukemia and myelodysplastic syndrome .
	manualset3
95773	3	400727	13	NULL	NULL	0	NULL	50 adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study we estimated serum GlcNAc-phosphotransferase in 50 adults suffering from leukemia and myelodysplastic syndrome .
	manualset3
95774	4	400727	13	NULL	NULL	0	NULL	suffering 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study we estimated serum GlcNAc-phosphotransferase in 50 adults suffering from leukemia and myelodysplastic syndrome .
	manualset3
95775	5	400727	13	NULL	NULL	0	NULL	 leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study we estimated serum GlcNAc-phosphotransferase in 50 adults suffering from leukemia and myelodysplastic syndrome .
	manualset3
95776	6	400727	13	NULL	NULL	0	NULL	myelodysplastic syndrome 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study we estimated serum GlcNAc-phosphotransferase in 50 adults suffering from leukemia and myelodysplastic syndrome .
	manualset3
95777	1	400728	13	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study we investigated the adipogenic differentiation properties of four human iPS cell lines and compared them with those of two human embryonic stem ( ES ) cell lines .
	manualset3
95778	2	400728	13	NULL	NULL	0	NULL	adipogenic differentiation properties	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study we investigated the adipogenic differentiation properties of four human iPS cell lines and compared them with those of two human embryonic stem ( ES ) cell lines .
	manualset3
95779	3	400728	13	NULL	NULL	0	NULL	four	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study we investigated the adipogenic differentiation properties of four human iPS cell lines and compared them with those of two human embryonic stem ( ES ) cell lines .
	manualset3
95780	4	400728	13	NULL	NULL	0	NULL	human iPS cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study we investigated the adipogenic differentiation properties of four human iPS cell lines and compared them with those of two human embryonic stem ( ES ) cell lines .
	manualset3
95781	5	400728	13	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study we investigated the adipogenic differentiation properties of four human iPS cell lines and compared them with those of two human embryonic stem ( ES ) cell lines .
	manualset3
95782	6	400728	13	NULL	NULL	0	NULL	human embryonic stem ( ES ) cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study we investigated the adipogenic differentiation properties of four human iPS cell lines and compared them with those of two human embryonic stem ( ES ) cell lines .
	manualset3
95783	1	400729	13	NULL	NULL	0	NULL	present work 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present work , we isolated two bioactive diterpenoids , horminone and 7-O-acetylhorminone and developed a micellar electrokinetic chromatography ( MEKC ) method for the simultaneous quantitative analysis of them in Turkish Salvia species .
	manualset3
95784	2	400729	13	NULL	NULL	0	NULL	two bioactive diterpenoids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present work , we isolated two bioactive diterpenoids , horminone and 7-O-acetylhorminone and developed a micellar electrokinetic chromatography ( MEKC ) method for the simultaneous quantitative analysis of them in Turkish Salvia species .
	manualset3
95785	3	400729	13	NULL	NULL	0	NULL	horminone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present work , we isolated two bioactive diterpenoids , horminone and 7-O-acetylhorminone and developed a micellar electrokinetic chromatography ( MEKC ) method for the simultaneous quantitative analysis of them in Turkish Salvia species .
	manualset3
95786	4	400729	13	NULL	NULL	0	NULL	7-O-acetylhorminone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present work , we isolated two bioactive diterpenoids , horminone and 7-O-acetylhorminone and developed a micellar electrokinetic chromatography ( MEKC ) method for the simultaneous quantitative analysis of them in Turkish Salvia species .
	manualset3
95787	5	400729	13	NULL	NULL	0	NULL	micellar electrokinetic chromatography ( MEKC ) method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present work , we isolated two bioactive diterpenoids , horminone and 7-O-acetylhorminone and developed a micellar electrokinetic chromatography ( MEKC ) method for the simultaneous quantitative analysis of them in Turkish Salvia species .
	manualset3
95788	6	400729	13	NULL	NULL	0	NULL	simultaneous quantitative analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present work , we isolated two bioactive diterpenoids , horminone and 7-O-acetylhorminone and developed a micellar electrokinetic chromatography ( MEKC ) method for the simultaneous quantitative analysis of them in Turkish Salvia species .
	manualset3
95789	7	400729	13	NULL	NULL	0	NULL	Turkish Salvia species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present work , we isolated two bioactive diterpenoids , horminone and 7-O-acetylhorminone and developed a micellar electrokinetic chromatography ( MEKC ) method for the simultaneous quantitative analysis of them in Turkish Salvia species .
	manualset3
95790	1	400730	13	NULL	NULL	0	NULL	primary motor cortex 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the primary motor cortex of PSP cases , neuronal loss was confined to inhibitory interneurones , whereas in the pre-SMA both interneurones ( reduced by 26 % ) and corticocortical projection neurones ( reduced by 82 % ) were affected .
	manualset3
95791	2	400730	13	NULL	NULL	0	NULL	PSP cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the primary motor cortex of PSP cases , neuronal loss was confined to inhibitory interneurones , whereas in the pre-SMA both interneurones ( reduced by 26 % ) and corticocortical projection neurones ( reduced by 82 % ) were affected .
	manualset3
95792	3	400730	13	NULL	NULL	0	NULL	neuronal loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the primary motor cortex of PSP cases , neuronal loss was confined to inhibitory interneurones , whereas in the pre-SMA both interneurones ( reduced by 26 % ) and corticocortical projection neurones ( reduced by 82 % ) were affected .
	manualset3
95793	4	400730	13	NULL	NULL	0	NULL	nhibitory interneurones	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the primary motor cortex of PSP cases , neuronal loss was confined to inhibitory interneurones , whereas in the pre-SMA both interneurones ( reduced by 26 % ) and corticocortical projection neurones ( reduced by 82 % ) were affected .
	manualset3
95794	5	400730	13	NULL	NULL	0	NULL	pre-SMA	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the primary motor cortex of PSP cases , neuronal loss was confined to inhibitory interneurones , whereas in the pre-SMA both interneurones ( reduced by 26 % ) and corticocortical projection neurones ( reduced by 82 % ) were affected .
	manualset3
95795	6	400730	13	NULL	NULL	0	NULL	interneurones	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the primary motor cortex of PSP cases , neuronal loss was confined to inhibitory interneurones , whereas in the pre-SMA both interneurones ( reduced by 26 % ) and corticocortical projection neurones ( reduced by 82 % ) were affected .
	manualset3
95796	7	400730	13	NULL	NULL	0	NULL	reduced by 26 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the primary motor cortex of PSP cases , neuronal loss was confined to inhibitory interneurones , whereas in the pre-SMA both interneurones ( reduced by 26 % ) and corticocortical projection neurones ( reduced by 82 % ) were affected .
	manualset3
95797	8	400730	13	NULL	NULL	0	NULL	projection neurones	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the primary motor cortex of PSP cases , neuronal loss was confined to inhibitory interneurones , whereas in the pre-SMA both interneurones ( reduced by 26 % ) and corticocortical projection neurones ( reduced by 82 % ) were affected .
	manualset3
95798	9	400730	13	NULL	NULL	0	NULL	 reduced by 82 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the primary motor cortex of PSP cases , neuronal loss was confined to inhibitory interneurones , whereas in the pre-SMA both interneurones ( reduced by 26 % ) and corticocortical projection neurones ( reduced by 82 % ) were affected .
	manualset3
95893	1	400731	13	NULL	NULL	NULL	NULL	prior bisphosphonate groups	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the prior bisphosphonate and bisphosphonate naive groups , respectively , the change in spinal BMD was 9.0 % and 7.8 % ( P = 0.54 ) at 12 months and 9.8 % and 6.1 % ( P = 0.30 ) at 18 months .
	manualset3
95895	2	400731	13	NULL	NULL	0	NULL	bisphosphonate naive groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the prior bisphosphonate and bisphosphonate naive groups , respectively , the change in spinal BMD was 9.0 % and 7.8 % ( P = 0.54 ) at 12 months and 9.8 % and 6.1 % ( P = 0.30 ) at 18 months .
	manualset3
95896	3	400731	13	NULL	NULL	0	NULL	change in spinal BMD	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the prior bisphosphonate and bisphosphonate naive groups , respectively , the change in spinal BMD was 9.0 % and 7.8 % ( P = 0.54 ) at 12 months and 9.8 % and 6.1 % ( P = 0.30 ) at 18 months .
	manualset3
95897	4	400731	13	NULL	NULL	0	NULL	9.0 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the prior bisphosphonate and bisphosphonate naive groups , respectively , the change in spinal BMD was 9.0 % and 7.8 % ( P = 0.54 ) at 12 months and 9.8 % and 6.1 % ( P = 0.30 ) at 18 months .
	manualset3
95898	5	400731	13	NULL	NULL	0	NULL	 7.8 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the prior bisphosphonate and bisphosphonate naive groups , respectively , the change in spinal BMD was 9.0 % and 7.8 % ( P = 0.54 ) at 12 months and 9.8 % and 6.1 % ( P = 0.30 ) at 18 months .
	manualset3
95899	6	400731	13	NULL	NULL	0	NULL	P = 0.54 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the prior bisphosphonate and bisphosphonate naive groups , respectively , the change in spinal BMD was 9.0 % and 7.8 % ( P = 0.54 ) at 12 months and 9.8 % and 6.1 % ( P = 0.30 ) at 18 months .
	manualset3
95900	7	400731	13	NULL	NULL	0	NULL	12 months	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In the prior bisphosphonate and bisphosphonate naive groups , respectively , the change in spinal BMD was 9.0 % and 7.8 % ( P = 0.54 ) at 12 months and 9.8 % and 6.1 % ( P = 0.30 ) at 18 months .
	manualset3
95901	8	400731	13	NULL	NULL	0	NULL	9.8 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the prior bisphosphonate and bisphosphonate naive groups , respectively , the change in spinal BMD was 9.0 % and 7.8 % ( P = 0.54 ) at 12 months and 9.8 % and 6.1 % ( P = 0.30 ) at 18 months .
	manualset3
95902	9	400731	13	NULL	NULL	0	NULL	 6.1 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the prior bisphosphonate and bisphosphonate naive groups , respectively , the change in spinal BMD was 9.0 % and 7.8 % ( P = 0.54 ) at 12 months and 9.8 % and 6.1 % ( P = 0.30 ) at 18 months .
	manualset3
95903	10	400731	13	NULL	NULL	0	NULL	 P = 0.30	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the prior bisphosphonate and bisphosphonate naive groups , respectively , the change in spinal BMD was 9.0 % and 7.8 % ( P = 0.54 ) at 12 months and 9.8 % and 6.1 % ( P = 0.30 ) at 18 months .
	manualset3
95904	11	400731	13	NULL	NULL	0	NULL	18 months  	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In the prior bisphosphonate and bisphosphonate naive groups , respectively , the change in spinal BMD was 9.0 % and 7.8 % ( P = 0.54 ) at 12 months and 9.8 % and 6.1 % ( P = 0.30 ) at 18 months .
	manualset3
95905	1	400732	13	NULL	NULL	0	NULL	prostate	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the prostate , the Nkx3 .1 homeobox gene plays an important role in normal differentiation of the prostatic epithelium while its loss of function is an initiating event in prostate carcinogenesis in both mouse models and human patients .
	manualset3
95906	2	400732	13	NULL	NULL	0	NULL	Nkx3 .1 homeobox gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In the prostate , the Nkx3 .1 homeobox gene plays an important role in normal differentiation of the prostatic epithelium while its loss of function is an initiating event in prostate carcinogenesis in both mouse models and human patients .
	manualset3
95907	3	400732	13	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the prostate , the Nkx3 .1 homeobox gene plays an important role in normal differentiation of the prostatic epithelium while its loss of function is an initiating event in prostate carcinogenesis in both mouse models and human patients .
	manualset3
95908	4	400732	13	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the prostate , the Nkx3 .1 homeobox gene plays an important role in normal differentiation of the prostatic epithelium while its loss of function is an initiating event in prostate carcinogenesis in both mouse models and human patients .
	manualset3
95909	5	400732	13	NULL	NULL	0	NULL	prostatic epithelium 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In the prostate , the Nkx3 .1 homeobox gene plays an important role in normal differentiation of the prostatic epithelium while its loss of function is an initiating event in prostate carcinogenesis in both mouse models and human patients .
	manualset3
95910	6	400732	13	NULL	NULL	0	NULL	 loss	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the prostate , the Nkx3 .1 homeobox gene plays an important role in normal differentiation of the prostatic epithelium while its loss of function is an initiating event in prostate carcinogenesis in both mouse models and human patients .
	manualset3
95911	7	400732	13	NULL	NULL	0	NULL	function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the prostate , the Nkx3 .1 homeobox gene plays an important role in normal differentiation of the prostatic epithelium while its loss of function is an initiating event in prostate carcinogenesis in both mouse models and human patients .
	manualset3
95912	8	400732	13	NULL	NULL	0	NULL	event 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the prostate , the Nkx3 .1 homeobox gene plays an important role in normal differentiation of the prostatic epithelium while its loss of function is an initiating event in prostate carcinogenesis in both mouse models and human patients .
	manualset3
95913	9	400732	13	NULL	NULL	0	NULL	prostate carcinogenesis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the prostate , the Nkx3 .1 homeobox gene plays an important role in normal differentiation of the prostatic epithelium while its loss of function is an initiating event in prostate carcinogenesis in both mouse models and human patients .
	manualset3
95914	10	400732	13	NULL	NULL	0	NULL	mouse models 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the prostate , the Nkx3 .1 homeobox gene plays an important role in normal differentiation of the prostatic epithelium while its loss of function is an initiating event in prostate carcinogenesis in both mouse models and human patients .
	manualset3
95915	11	400732	13	NULL	NULL	0	NULL	 human patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the prostate , the Nkx3 .1 homeobox gene plays an important role in normal differentiation of the prostatic epithelium while its loss of function is an initiating event in prostate carcinogenesis in both mouse models and human patients .
	manualset3
95916	1	400733	13	NULL	NULL	0	NULL	race 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the race to provide the patient population with effective treatment systems , filtration technologies are playing a greater role in meeting the challenges .
	manualset3
95917	2	400733	13	NULL	NULL	0	NULL	patient population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the race to provide the patient population with effective treatment systems , filtration technologies are playing a greater role in meeting the challenges .
	manualset3
95918	3	400733	13	NULL	NULL	0	NULL	 effective treatment systems	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the race to provide the patient population with effective treatment systems , filtration technologies are playing a greater role in meeting the challenges .
	manualset3
95919	4	400733	13	NULL	NULL	0	NULL	 filtration technologies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the race to provide the patient population with effective treatment systems , filtration technologies are playing a greater role in meeting the challenges .
	manualset3
95920	5	400733	13	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the race to provide the patient population with effective treatment systems , filtration technologies are playing a greater role in meeting the challenges .
	manualset3
95921	6	400733	13	NULL	NULL	0	NULL	challenges	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the race to provide the patient population with effective treatment systems , filtration technologies are playing a greater role in meeting the challenges .
	manualset3
95922	1	400734	13	NULL	NULL	0	NULL	 range of 1-8 units 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the range of 1-8 units the precision of choice in pigeons depended on absolute and relative differences between comparing values .
	manualset3
95923	2	400734	13	NULL	NULL	0	NULL	precision 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the range of 1-8 units the precision of choice in pigeons depended on absolute and relative differences between comparing values .
	manualset3
95924	3	400734	13	NULL	NULL	0	NULL	choice 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the range of 1-8 units the precision of choice in pigeons depended on absolute and relative differences between comparing values .
	manualset3
95925	4	400734	13	NULL	NULL	0	NULL	 pigeons	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the range of 1-8 units the precision of choice in pigeons depended on absolute and relative differences between comparing values .
	manualset3
95926	5	400734	13	NULL	NULL	0	NULL	absolute differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In the range of 1-8 units the precision of choice in pigeons depended on absolute and relative differences between comparing values .
	manualset3
95927	6	400734	13	NULL	NULL	0	NULL	relative differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In the range of 1-8 units the precision of choice in pigeons depended on absolute and relative differences between comparing values .
	manualset3
95928	7	400734	13	NULL	NULL	0	NULL	values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the range of 1-8 units the precision of choice in pigeons depended on absolute and relative differences between comparing values .
	manualset3
95929	1	400735	13	NULL	NULL	0	NULL	108 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	108 patients with T2 or T3 carcinoma of the bladder were randomised to receive either photon therapy or low - or high-dose 15 MeV neutrons .
	manualset3
95930	2	400735	13	NULL	NULL	0	NULL	T2 carcinoma of the bladder 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	108 patients with T2 or T3 carcinoma of the bladder were randomised to receive either photon therapy or low - or high-dose 15 MeV neutrons .
	manualset3
95931	3	400735	13	NULL	NULL	0	NULL	T3 carcinoma of the bladder 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	108 patients with T2 or T3 carcinoma of the bladder were randomised to receive either photon therapy or low - or high-dose 15 MeV neutrons .
	manualset3
95932	4	400735	13	NULL	NULL	0	NULL	 photon therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	108 patients with T2 or T3 carcinoma of the bladder were randomised to receive either photon therapy or low - or high-dose 15 MeV neutrons .
	manualset3
95933	5	400735	13	NULL	NULL	0	NULL	high-dose 15 MeV neutrons	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	108 patients with T2 or T3 carcinoma of the bladder were randomised to receive either photon therapy or low - or high-dose 15 MeV neutrons .
	manualset3
95934	6	400735	13	NULL	NULL	0	NULL	low -dose 15 MeV neutrons 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	108 patients with T2 or T3 carcinoma of the bladder were randomised to receive either photon therapy or low - or high-dose 15 MeV neutrons .
	manualset3
95935	1	400736	13	NULL	NULL	0	NULL	b-c1 complex 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the reconstituted b-c1 complex , dicyclohexylcarbodiimide ( DCCD ) blocked the function of the electrogenic proton translocating device in the forward direction of proton ejection as well as in the backwards direction , measured as reversed electron flow from cytochrome b to coenzyme Q2 driven by a K + - diffusion potential .
	manualset3
95936	2	400736	13	NULL	NULL	0	NULL	dicyclohexylcarbodiimide ( DCCD )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the reconstituted b-c1 complex , dicyclohexylcarbodiimide ( DCCD ) blocked the function of the electrogenic proton translocating device in the forward direction of proton ejection as well as in the backwards direction , measured as reversed electron flow from cytochrome b to coenzyme Q2 driven by a K + - diffusion potential .
	manualset3
95937	3	400736	13	NULL	NULL	0	NULL	 function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the reconstituted b-c1 complex , dicyclohexylcarbodiimide ( DCCD ) blocked the function of the electrogenic proton translocating device in the forward direction of proton ejection as well as in the backwards direction , measured as reversed electron flow from cytochrome b to coenzyme Q2 driven by a K + - diffusion potential .
	manualset3
95938	4	400736	13	NULL	NULL	0	NULL	electrogenic proton translocating device 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In the reconstituted b-c1 complex , dicyclohexylcarbodiimide ( DCCD ) blocked the function of the electrogenic proton translocating device in the forward direction of proton ejection as well as in the backwards direction , measured as reversed electron flow from cytochrome b to coenzyme Q2 driven by a K + - diffusion potential .
	manualset3
95939	5	400736	13	NULL	NULL	NULL	NULL	forward direction	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the reconstituted b-c1 complex , dicyclohexylcarbodiimide ( DCCD ) blocked the function of the electrogenic proton translocating device in the forward direction of proton ejection as well as in the backwards direction , measured as reversed electron flow from cytochrome b to coenzyme Q2 driven by a K + - diffusion potential .
	manualset3
95940	6	400736	13	NULL	NULL	0	NULL	proton ejection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the reconstituted b-c1 complex , dicyclohexylcarbodiimide ( DCCD ) blocked the function of the electrogenic proton translocating device in the forward direction of proton ejection as well as in the backwards direction , measured as reversed electron flow from cytochrome b to coenzyme Q2 driven by a K + - diffusion potential .
	manualset3
95941	7	400736	13	NULL	NULL	NULL	NULL	backwards direction	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the reconstituted b-c1 complex , dicyclohexylcarbodiimide ( DCCD ) blocked the function of the electrogenic proton translocating device in the forward direction of proton ejection as well as in the backwards direction , measured as reversed electron flow from cytochrome b to coenzyme Q2 driven by a K + - diffusion potential .
	manualset3
95942	8	400736	13	NULL	NULL	0	NULL	electron flow 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the reconstituted b-c1 complex , dicyclohexylcarbodiimide ( DCCD ) blocked the function of the electrogenic proton translocating device in the forward direction of proton ejection as well as in the backwards direction , measured as reversed electron flow from cytochrome b to coenzyme Q2 driven by a K + - diffusion potential .
	manualset3
95943	9	400736	13	NULL	NULL	0	NULL	cytochrome b	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the reconstituted b-c1 complex , dicyclohexylcarbodiimide ( DCCD ) blocked the function of the electrogenic proton translocating device in the forward direction of proton ejection as well as in the backwards direction , measured as reversed electron flow from cytochrome b to coenzyme Q2 driven by a K + - diffusion potential .
	manualset3
95944	10	400736	13	NULL	NULL	0	NULL	coenzyme Q2	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the reconstituted b-c1 complex , dicyclohexylcarbodiimide ( DCCD ) blocked the function of the electrogenic proton translocating device in the forward direction of proton ejection as well as in the backwards direction , measured as reversed electron flow from cytochrome b to coenzyme Q2 driven by a K + - diffusion potential .
	manualset3
95945	11	400736	13	NULL	NULL	0	NULL	K + - diffusion potential	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the reconstituted b-c1 complex , dicyclohexylcarbodiimide ( DCCD ) blocked the function of the electrogenic proton translocating device in the forward direction of proton ejection as well as in the backwards direction , measured as reversed electron flow from cytochrome b to coenzyme Q2 driven by a K + - diffusion potential .
	manualset3
95946	1	400737	13	NULL	NULL	0	NULL	recurrent nerve 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the recurrent nerve , the fibers of the lateral part of the anterior lateral line ganglion terminated throughout the entire dorsal nucleus , and the fibers of the intracapsular ganglion projected to the dorsolateral part of the nucleus .
	manualset3
95947	2	400737	13	NULL	NULL	0	NULL	 fibers of the lateral part of the anterior lateral line ganglion	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the recurrent nerve , the fibers of the lateral part of the anterior lateral line ganglion terminated throughout the entire dorsal nucleus , and the fibers of the intracapsular ganglion projected to the dorsolateral part of the nucleus .
	manualset3
95948	3	400737	13	NULL	NULL	0	NULL	dorsal nucleus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the recurrent nerve , the fibers of the lateral part of the anterior lateral line ganglion terminated throughout the entire dorsal nucleus , and the fibers of the intracapsular ganglion projected to the dorsolateral part of the nucleus .
	manualset3
95949	4	400737	13	NULL	NULL	0	NULL	fibers of the intracapsular ganglion	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the recurrent nerve , the fibers of the lateral part of the anterior lateral line ganglion terminated throughout the entire dorsal nucleus , and the fibers of the intracapsular ganglion projected to the dorsolateral part of the nucleus .
	manualset3
95950	5	400737	13	NULL	NULL	0	NULL	dorsolateral part of the nucleus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the recurrent nerve , the fibers of the lateral part of the anterior lateral line ganglion terminated throughout the entire dorsal nucleus , and the fibers of the intracapsular ganglion projected to the dorsolateral part of the nucleus .
	manualset3
95951	1	400738	13	NULL	NULL	0	NULL	 three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the remaining three children , hepatitis B virus DNA could not be demonstrated in the tumor tissues .
	manualset3
95952	2	400738	13	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the remaining three children , hepatitis B virus DNA could not be demonstrated in the tumor tissues .
	manualset3
95953	3	400738	13	NULL	NULL	0	NULL	hepatitis B virus DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the remaining three children , hepatitis B virus DNA could not be demonstrated in the tumor tissues .
	manualset3
95954	4	400738	13	NULL	NULL	0	NULL	tumor tissues 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In the remaining three children , hepatitis B virus DNA could not be demonstrated in the tumor tissues .
	manualset3
95955	1	400739	13	NULL	NULL	0	NULL	respiratory chain	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the respiratory chain free energy is conserved by linking the chemical reduction of dioxygen to the electrogenic translocation of protons across a membrane .
	manualset3
95956	2	400739	13	NULL	NULL	0	NULL	free energy	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the respiratory chain free energy is conserved by linking the chemical reduction of dioxygen to the electrogenic translocation of protons across a membrane .
	manualset3
95957	3	400739	13	NULL	NULL	0	NULL	chemical reduction of dioxygen	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the respiratory chain free energy is conserved by linking the chemical reduction of dioxygen to the electrogenic translocation of protons across a membrane .
	manualset3
95958	4	400739	13	NULL	NULL	0	NULL	electrogenic translocation of protons 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the respiratory chain free energy is conserved by linking the chemical reduction of dioxygen to the electrogenic translocation of protons across a membrane .
	manualset3
95959	5	400739	13	NULL	NULL	0	NULL	 membrane	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the respiratory chain free energy is conserved by linking the chemical reduction of dioxygen to the electrogenic translocation of protons across a membrane .
	manualset3
95960	1	400740	13	NULL	NULL	0	NULL	 literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the revised literature , purine analog have been identified as the treatment of choice for this disease .
	manualset3
95961	2	400740	13	NULL	NULL	0	NULL	purine analog	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the revised literature , purine analog have been identified as the treatment of choice for this disease .
	manualset3
95962	3	400740	13	NULL	NULL	NULL	NULL	treatment of choice	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the revised literature , purine analog have been identified as the treatment of choice for this disease .
	manualset3
95963	4	400740	13	NULL	NULL	0	NULL	 disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In the revised literature , purine analog have been identified as the treatment of choice for this disease .
	manualset3
95964	1	400741	13	NULL	NULL	0	NULL	case of monomelic cancerous metastasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Apropos of a case of monomelic cancerous metastasis of the lower extremity ) .
	manualset3
95965	2	400741	13	NULL	NULL	0	NULL	lower extremity	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Apropos of a case of monomelic cancerous metastasis of the lower extremity ) .
	manualset3
95966	1	400742	13	NULL	NULL	0	NULL	11 beta-hydroxysteroid dehydrogenase ( 11 beta-HSD )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	11 beta-hydroxysteroid dehydrogenase ( 11 beta-HSD ) catalyzes the interconversion of cortisol ( F ) to inactive cortisone ( E ) in man ( corticosterone ( B ) to 11-dehydrocorticosterone ( A ) in rodents ) and plays a crucial role in regulating corticosteroid hormone action .
	manualset3
95967	2	400742	13	NULL	NULL	0	NULL	interconversion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	11 beta-hydroxysteroid dehydrogenase ( 11 beta-HSD ) catalyzes the interconversion of cortisol ( F ) to inactive cortisone ( E ) in man ( corticosterone ( B ) to 11-dehydrocorticosterone ( A ) in rodents ) and plays a crucial role in regulating corticosteroid hormone action .
	manualset3
95968	3	400742	13	NULL	NULL	0	NULL	 cortisol ( F )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	11 beta-hydroxysteroid dehydrogenase ( 11 beta-HSD ) catalyzes the interconversion of cortisol ( F ) to inactive cortisone ( E ) in man ( corticosterone ( B ) to 11-dehydrocorticosterone ( A ) in rodents ) and plays a crucial role in regulating corticosteroid hormone action .
	manualset3
95969	4	400742	13	NULL	NULL	0	NULL	cortisone ( E ) 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	11 beta-hydroxysteroid dehydrogenase ( 11 beta-HSD ) catalyzes the interconversion of cortisol ( F ) to inactive cortisone ( E ) in man ( corticosterone ( B ) to 11-dehydrocorticosterone ( A ) in rodents ) and plays a crucial role in regulating corticosteroid hormone action .
	manualset3
95970	5	400742	13	NULL	NULL	0	NULL	man 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	11 beta-hydroxysteroid dehydrogenase ( 11 beta-HSD ) catalyzes the interconversion of cortisol ( F ) to inactive cortisone ( E ) in man ( corticosterone ( B ) to 11-dehydrocorticosterone ( A ) in rodents ) and plays a crucial role in regulating corticosteroid hormone action .
	manualset3
95971	6	400742	13	NULL	NULL	0	NULL	corticosterone ( B ) 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	11 beta-hydroxysteroid dehydrogenase ( 11 beta-HSD ) catalyzes the interconversion of cortisol ( F ) to inactive cortisone ( E ) in man ( corticosterone ( B ) to 11-dehydrocorticosterone ( A ) in rodents ) and plays a crucial role in regulating corticosteroid hormone action .
	manualset3
95972	7	400742	13	NULL	NULL	0	NULL	11-dehydrocorticosterone ( A )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	11 beta-hydroxysteroid dehydrogenase ( 11 beta-HSD ) catalyzes the interconversion of cortisol ( F ) to inactive cortisone ( E ) in man ( corticosterone ( B ) to 11-dehydrocorticosterone ( A ) in rodents ) and plays a crucial role in regulating corticosteroid hormone action .
	manualset3
95973	8	400742	13	NULL	NULL	0	NULL	rodents 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	11 beta-hydroxysteroid dehydrogenase ( 11 beta-HSD ) catalyzes the interconversion of cortisol ( F ) to inactive cortisone ( E ) in man ( corticosterone ( B ) to 11-dehydrocorticosterone ( A ) in rodents ) and plays a crucial role in regulating corticosteroid hormone action .
	manualset3
95974	9	400742	13	NULL	NULL	0	NULL	crucial role 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	11 beta-hydroxysteroid dehydrogenase ( 11 beta-HSD ) catalyzes the interconversion of cortisol ( F ) to inactive cortisone ( E ) in man ( corticosterone ( B ) to 11-dehydrocorticosterone ( A ) in rodents ) and plays a crucial role in regulating corticosteroid hormone action .
	manualset3
95975	10	400742	13	NULL	NULL	0	NULL	corticosteroid hormone action 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	11 beta-hydroxysteroid dehydrogenase ( 11 beta-HSD ) catalyzes the interconversion of cortisol ( F ) to inactive cortisone ( E ) in man ( corticosterone ( B ) to 11-dehydrocorticosterone ( A ) in rodents ) and plays a crucial role in regulating corticosteroid hormone action .
	manualset3
95976	1	400743	13	NULL	NULL	0	NULL	 saline control group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the saline control group the remarkable inhibitory effect of EA was observed 0 ' -8 ' after ceasing EA , The results showed that the inhibitory effect of EA in the test group was weaker than that in the control group .
	manualset3
95977	2	400743	13	NULL	NULL	NULL	NULL	 inhibitory effect	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the saline control group the remarkable inhibitory effect of EA was observed 0 ' -8 ' after ceasing EA , The results showed that the inhibitory effect of EA in the test group was weaker than that in the control group .
	manualset3
95978	3	400743	13	NULL	NULL	0	NULL	EA 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the saline control group the remarkable inhibitory effect of EA was observed 0 ' -8 ' after ceasing EA , The results showed that the inhibitory effect of EA in the test group was weaker than that in the control group .
	manualset3
95979	4	400743	13	NULL	NULL	0	NULL	0 ' -8 '	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the saline control group the remarkable inhibitory effect of EA was observed 0 ' -8 ' after ceasing EA , The results showed that the inhibitory effect of EA in the test group was weaker than that in the control group .
	manualset3
95980	5	400743	13	NULL	NULL	0	NULL	EA 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the saline control group the remarkable inhibitory effect of EA was observed 0 ' -8 ' after ceasing EA , The results showed that the inhibitory effect of EA in the test group was weaker than that in the control group .
	manualset3
95981	6	400743	13	NULL	NULL	NULL	NULL	inhibitory effect	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the saline control group the remarkable inhibitory effect of EA was observed 0 ' -8 ' after ceasing EA , The results showed that the inhibitory effect of EA in the test group was weaker than that in the control group .
	manualset3
95982	7	400743	13	NULL	NULL	0	NULL	EA	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the saline control group the remarkable inhibitory effect of EA was observed 0 ' -8 ' after ceasing EA , The results showed that the inhibitory effect of EA in the test group was weaker than that in the control group .
	manualset3
95983	8	400743	13	NULL	NULL	0	NULL	 test group 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the saline control group the remarkable inhibitory effect of EA was observed 0 ' -8 ' after ceasing EA , The results showed that the inhibitory effect of EA in the test group was weaker than that in the control group .
	manualset3
95984	9	400743	13	NULL	NULL	0	NULL	 control group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the saline control group the remarkable inhibitory effect of EA was observed 0 ' -8 ' after ceasing EA , The results showed that the inhibitory effect of EA in the test group was weaker than that in the control group .
	manualset3
95985	1	400744	13	NULL	NULL	NULL	NULL	screening process 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the screening process , each risk factor was evaluated as a single fixed effects factor in a multilevel model that accounted for variability among the sampled farms and their production complexes and companies .
	manualset3
95986	2	400744	13	NULL	NULL	0	NULL	risk factor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the screening process , each risk factor was evaluated as a single fixed effects factor in a multilevel model that accounted for variability among the sampled farms and their production complexes and companies .
	manualset3
95987	3	400744	13	NULL	NULL	0	NULL	effects factor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the screening process , each risk factor was evaluated as a single fixed effects factor in a multilevel model that accounted for variability among the sampled farms and their production complexes and companies .
	manualset3
95988	4	400744	13	NULL	NULL	0	NULL	multilevel model	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In the screening process , each risk factor was evaluated as a single fixed effects factor in a multilevel model that accounted for variability among the sampled farms and their production complexes and companies .
	manualset3
95989	5	400744	13	NULL	NULL	0	NULL	variability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the screening process , each risk factor was evaluated as a single fixed effects factor in a multilevel model that accounted for variability among the sampled farms and their production complexes and companies .
	manualset3
95990	6	400744	13	NULL	NULL	0	NULL	sampled farms	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In the screening process , each risk factor was evaluated as a single fixed effects factor in a multilevel model that accounted for variability among the sampled farms and their production complexes and companies .
	manualset3
95991	7	400744	13	NULL	NULL	0	NULL	production complexes 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the screening process , each risk factor was evaluated as a single fixed effects factor in a multilevel model that accounted for variability among the sampled farms and their production complexes and companies .
	manualset3
95992	8	400744	13	NULL	NULL	0	NULL	companies	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In the screening process , each risk factor was evaluated as a single fixed effects factor in a multilevel model that accounted for variability among the sampled farms and their production complexes and companies .
	manualset3
95993	1	400745	13	NULL	NULL	0	NULL	sea area	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the sea area , there existed remarkable differences in the accumulation and degradation of HCH and DDT among different shellfish culture environments , being mostly associated with the habitation environment and physiological life habits of shellfish .
	manualset3
95994	2	400745	13	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In the sea area , there existed remarkable differences in the accumulation and degradation of HCH and DDT among different shellfish culture environments , being mostly associated with the habitation environment and physiological life habits of shellfish .
	manualset3
95995	3	400745	13	NULL	NULL	0	NULL	 accumulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the sea area , there existed remarkable differences in the accumulation and degradation of HCH and DDT among different shellfish culture environments , being mostly associated with the habitation environment and physiological life habits of shellfish .
	manualset3
95996	4	400745	13	NULL	NULL	0	NULL	degradation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the sea area , there existed remarkable differences in the accumulation and degradation of HCH and DDT among different shellfish culture environments , being mostly associated with the habitation environment and physiological life habits of shellfish .
	manualset3
95997	5	400745	13	NULL	NULL	0	NULL	HCH	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the sea area , there existed remarkable differences in the accumulation and degradation of HCH and DDT among different shellfish culture environments , being mostly associated with the habitation environment and physiological life habits of shellfish .
	manualset3
95998	6	400745	13	NULL	NULL	0	NULL	DDT 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the sea area , there existed remarkable differences in the accumulation and degradation of HCH and DDT among different shellfish culture environments , being mostly associated with the habitation environment and physiological life habits of shellfish .
	manualset3
95999	7	400745	13	NULL	NULL	0	NULL	 shellfish culture environments 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the sea area , there existed remarkable differences in the accumulation and degradation of HCH and DDT among different shellfish culture environments , being mostly associated with the habitation environment and physiological life habits of shellfish .
	manualset3
96000	8	400745	13	NULL	NULL	0	NULL	habitation environment	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the sea area , there existed remarkable differences in the accumulation and degradation of HCH and DDT among different shellfish culture environments , being mostly associated with the habitation environment and physiological life habits of shellfish .
	manualset3
96001	9	400745	13	NULL	NULL	0	NULL	physiological life habits	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the sea area , there existed remarkable differences in the accumulation and degradation of HCH and DDT among different shellfish culture environments , being mostly associated with the habitation environment and physiological life habits of shellfish .
	manualset3
96002	10	400745	13	NULL	NULL	0	NULL	shellfish	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the sea area , there existed remarkable differences in the accumulation and degradation of HCH and DDT among different shellfish culture environments , being mostly associated with the habitation environment and physiological life habits of shellfish .
	manualset3
96003	1	400746	13	NULL	NULL	0	NULL	search	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the search for any deleterious hemodynamic effects of the acute administration of intravenous diltiazem ( 0.25 mg/kg ) , in patients on beta blockers , studies were performed in two comparable groups of eight patients with chronic coronary heart disease without clinical signs of heart failure .
	manualset3
96004	2	400746	13	NULL	NULL	0	NULL	hemodynamic effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the search for any deleterious hemodynamic effects of the acute administration of intravenous diltiazem ( 0.25 mg/kg ) , in patients on beta blockers , studies were performed in two comparable groups of eight patients with chronic coronary heart disease without clinical signs of heart failure .
	manualset3
96005	3	400746	13	NULL	NULL	NULL	NULL	administration of intravenous diltiazem	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the search for any deleterious hemodynamic effects of the acute administration of intravenous diltiazem ( 0.25 mg/kg ) , in patients on beta blockers , studies were performed in two comparable groups of eight patients with chronic coronary heart disease without clinical signs of heart failure .
	manualset3
96006	4	400746	13	NULL	NULL	0	NULL	0.25 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the search for any deleterious hemodynamic effects of the acute administration of intravenous diltiazem ( 0.25 mg/kg ) , in patients on beta blockers , studies were performed in two comparable groups of eight patients with chronic coronary heart disease without clinical signs of heart failure .
	manualset3
96007	5	400746	13	NULL	NULL	0	NULL	 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the search for any deleterious hemodynamic effects of the acute administration of intravenous diltiazem ( 0.25 mg/kg ) , in patients on beta blockers , studies were performed in two comparable groups of eight patients with chronic coronary heart disease without clinical signs of heart failure .
	manualset3
96008	6	400746	13	NULL	NULL	0	NULL	 beta blockers	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the search for any deleterious hemodynamic effects of the acute administration of intravenous diltiazem ( 0.25 mg/kg ) , in patients on beta blockers , studies were performed in two comparable groups of eight patients with chronic coronary heart disease without clinical signs of heart failure .
	manualset3
96009	7	400746	13	NULL	NULL	0	NULL	 studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the search for any deleterious hemodynamic effects of the acute administration of intravenous diltiazem ( 0.25 mg/kg ) , in patients on beta blockers , studies were performed in two comparable groups of eight patients with chronic coronary heart disease without clinical signs of heart failure .
	manualset3
96010	8	400746	13	NULL	NULL	0	NULL	two comparable groups 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the search for any deleterious hemodynamic effects of the acute administration of intravenous diltiazem ( 0.25 mg/kg ) , in patients on beta blockers , studies were performed in two comparable groups of eight patients with chronic coronary heart disease without clinical signs of heart failure .
	manualset3
96011	9	400746	13	NULL	NULL	0	NULL	eight patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the search for any deleterious hemodynamic effects of the acute administration of intravenous diltiazem ( 0.25 mg/kg ) , in patients on beta blockers , studies were performed in two comparable groups of eight patients with chronic coronary heart disease without clinical signs of heart failure .
	manualset3
96012	10	400746	13	NULL	NULL	0	NULL	chronic coronary heart disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In the search for any deleterious hemodynamic effects of the acute administration of intravenous diltiazem ( 0.25 mg/kg ) , in patients on beta blockers , studies were performed in two comparable groups of eight patients with chronic coronary heart disease without clinical signs of heart failure .
	manualset3
96013	11	400746	13	NULL	NULL	0	NULL	clinical signs of heart failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the search for any deleterious hemodynamic effects of the acute administration of intravenous diltiazem ( 0.25 mg/kg ) , in patients on beta blockers , studies were performed in two comparable groups of eight patients with chronic coronary heart disease without clinical signs of heart failure .
	manualset3
96014	1	400747	13	NULL	NULL	0	NULL	search	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the search for the primary roots of autonomy ( a pivotal concept in Varela 's comprehensive understanding of living beings ) , the theory of autopoiesis provided an explicit criterion to define minimal life in universal terms , and was taken as a guideline in the research program for the artificial synthesis of biological systems .
	manualset3
96015	2	400747	13	NULL	NULL	0	NULL	primary roots of autonomy 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In the search for the primary roots of autonomy ( a pivotal concept in Varela 's comprehensive understanding of living beings ) , the theory of autopoiesis provided an explicit criterion to define minimal life in universal terms , and was taken as a guideline in the research program for the artificial synthesis of biological systems .
	manualset3
96016	3	400747	13	NULL	NULL	0	NULL	pivotal concept	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In the search for the primary roots of autonomy ( a pivotal concept in Varela 's comprehensive understanding of living beings ) , the theory of autopoiesis provided an explicit criterion to define minimal life in universal terms , and was taken as a guideline in the research program for the artificial synthesis of biological systems .
	manualset3
96017	4	400747	13	NULL	NULL	0	NULL	Varela 's	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In the search for the primary roots of autonomy ( a pivotal concept in Varela 's comprehensive understanding of living beings ) , the theory of autopoiesis provided an explicit criterion to define minimal life in universal terms , and was taken as a guideline in the research program for the artificial synthesis of biological systems .
	manualset3
96018	5	400747	13	NULL	NULL	0	NULL	understanding 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the search for the primary roots of autonomy ( a pivotal concept in Varela 's comprehensive understanding of living beings ) , the theory of autopoiesis provided an explicit criterion to define minimal life in universal terms , and was taken as a guideline in the research program for the artificial synthesis of biological systems .
	manualset3
96019	6	400747	13	NULL	NULL	0	NULL	living beings	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the search for the primary roots of autonomy ( a pivotal concept in Varela 's comprehensive understanding of living beings ) , the theory of autopoiesis provided an explicit criterion to define minimal life in universal terms , and was taken as a guideline in the research program for the artificial synthesis of biological systems .
	manualset3
96020	7	400747	13	NULL	NULL	0	NULL	theory of autopoiesis 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In the search for the primary roots of autonomy ( a pivotal concept in Varela 's comprehensive understanding of living beings ) , the theory of autopoiesis provided an explicit criterion to define minimal life in universal terms , and was taken as a guideline in the research program for the artificial synthesis of biological systems .
	manualset3
96021	8	400747	13	NULL	NULL	0	NULL	 criterion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the search for the primary roots of autonomy ( a pivotal concept in Varela 's comprehensive understanding of living beings ) , the theory of autopoiesis provided an explicit criterion to define minimal life in universal terms , and was taken as a guideline in the research program for the artificial synthesis of biological systems .
	manualset3
96022	9	400747	13	NULL	NULL	0	NULL	minimal life 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the search for the primary roots of autonomy ( a pivotal concept in Varela 's comprehensive understanding of living beings ) , the theory of autopoiesis provided an explicit criterion to define minimal life in universal terms , and was taken as a guideline in the research program for the artificial synthesis of biological systems .
	manualset3
96023	10	400747	13	NULL	NULL	0	NULL	 universal terms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the search for the primary roots of autonomy ( a pivotal concept in Varela 's comprehensive understanding of living beings ) , the theory of autopoiesis provided an explicit criterion to define minimal life in universal terms , and was taken as a guideline in the research program for the artificial synthesis of biological systems .
	manualset3
96024	11	400747	13	NULL	NULL	0	NULL	guideline	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the search for the primary roots of autonomy ( a pivotal concept in Varela 's comprehensive understanding of living beings ) , the theory of autopoiesis provided an explicit criterion to define minimal life in universal terms , and was taken as a guideline in the research program for the artificial synthesis of biological systems .
	manualset3
96025	12	400747	13	NULL	NULL	0	NULL	research program 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the search for the primary roots of autonomy ( a pivotal concept in Varela 's comprehensive understanding of living beings ) , the theory of autopoiesis provided an explicit criterion to define minimal life in universal terms , and was taken as a guideline in the research program for the artificial synthesis of biological systems .
	manualset3
96026	13	400747	13	NULL	NULL	0	NULL	artificial synthesis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the search for the primary roots of autonomy ( a pivotal concept in Varela 's comprehensive understanding of living beings ) , the theory of autopoiesis provided an explicit criterion to define minimal life in universal terms , and was taken as a guideline in the research program for the artificial synthesis of biological systems .
	manualset3
96027	14	400747	13	NULL	NULL	0	NULL	biological systems	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the search for the primary roots of autonomy ( a pivotal concept in Varela 's comprehensive understanding of living beings ) , the theory of autopoiesis provided an explicit criterion to define minimal life in universal terms , and was taken as a guideline in the research program for the artificial synthesis of biological systems .
	manualset3
96028	1	400748	13	NULL	NULL	0	NULL	treatment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second , treatment of chlorofumaroyl dichloride with hydroxylamine also gave the intermediate chlorofumarodihydroxamic acid ( 6 ) .
	manualset3
96029	2	400748	13	NULL	NULL	0	NULL	chlorofumaroyl dichloride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second , treatment of chlorofumaroyl dichloride with hydroxylamine also gave the intermediate chlorofumarodihydroxamic acid ( 6 ) .
	manualset3
96030	3	400748	13	NULL	NULL	0	NULL	hydroxylamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second , treatment of chlorofumaroyl dichloride with hydroxylamine also gave the intermediate chlorofumarodihydroxamic acid ( 6 ) .
	manualset3
96031	4	400748	13	NULL	NULL	0	NULL	chlorofumarodihydroxamic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second , treatment of chlorofumaroyl dichloride with hydroxylamine also gave the intermediate chlorofumarodihydroxamic acid ( 6 ) .
	manualset3
96032	1	400749	13	NULL	NULL	0	NULL	biopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second biopsy the hsr and MLL amplification appears as nonreciprocal translocation of multiple copies in the form of marked amplification of MLL on chromosome 16 in a background of increasing chromosomal aberrations .
	manualset3
96033	2	400749	13	NULL	NULL	0	NULL	hsr	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second biopsy the hsr and MLL amplification appears as nonreciprocal translocation of multiple copies in the form of marked amplification of MLL on chromosome 16 in a background of increasing chromosomal aberrations .
	manualset3
96034	3	400749	13	NULL	NULL	0	NULL	MLL amplification 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second biopsy the hsr and MLL amplification appears as nonreciprocal translocation of multiple copies in the form of marked amplification of MLL on chromosome 16 in a background of increasing chromosomal aberrations .
	manualset3
96035	4	400749	13	NULL	NULL	0	NULL	nonreciprocal translocation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second biopsy the hsr and MLL amplification appears as nonreciprocal translocation of multiple copies in the form of marked amplification of MLL on chromosome 16 in a background of increasing chromosomal aberrations .
	manualset3
96036	5	400749	13	NULL	NULL	0	NULL	multiple copies 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second biopsy the hsr and MLL amplification appears as nonreciprocal translocation of multiple copies in the form of marked amplification of MLL on chromosome 16 in a background of increasing chromosomal aberrations .
	manualset3
96037	6	400749	13	NULL	NULL	0	NULL	 form	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second biopsy the hsr and MLL amplification appears as nonreciprocal translocation of multiple copies in the form of marked amplification of MLL on chromosome 16 in a background of increasing chromosomal aberrations .
	manualset3
96038	7	400749	13	NULL	NULL	0	NULL	amplification of MLL	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second biopsy the hsr and MLL amplification appears as nonreciprocal translocation of multiple copies in the form of marked amplification of MLL on chromosome 16 in a background of increasing chromosomal aberrations .
	manualset3
96039	8	400749	13	NULL	NULL	0	NULL	chromosome 16	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second biopsy the hsr and MLL amplification appears as nonreciprocal translocation of multiple copies in the form of marked amplification of MLL on chromosome 16 in a background of increasing chromosomal aberrations .
	manualset3
96040	9	400749	13	NULL	NULL	0	NULL	 chromosomal aberrations 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second biopsy the hsr and MLL amplification appears as nonreciprocal translocation of multiple copies in the form of marked amplification of MLL on chromosome 16 in a background of increasing chromosomal aberrations .
	manualset3
96041	1	400750	13	NULL	NULL	0	NULL	second example	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second example , a relationship was established between changes in membrane lipid composition during lung development and the activity of cholinephosphate cytidylyltransferase , the rate-limiting enzyme in phosphatidylcholine synthesis .
	manualset3
96042	2	400750	13	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second example , a relationship was established between changes in membrane lipid composition during lung development and the activity of cholinephosphate cytidylyltransferase , the rate-limiting enzyme in phosphatidylcholine synthesis .
	manualset3
96043	3	400750	13	NULL	NULL	0	NULL	changes 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second example , a relationship was established between changes in membrane lipid composition during lung development and the activity of cholinephosphate cytidylyltransferase , the rate-limiting enzyme in phosphatidylcholine synthesis .
	manualset3
96044	4	400750	13	NULL	NULL	0	NULL	membrane lipid composition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second example , a relationship was established between changes in membrane lipid composition during lung development and the activity of cholinephosphate cytidylyltransferase , the rate-limiting enzyme in phosphatidylcholine synthesis .
	manualset3
96045	5	400750	13	NULL	NULL	0	NULL	lung development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second example , a relationship was established between changes in membrane lipid composition during lung development and the activity of cholinephosphate cytidylyltransferase , the rate-limiting enzyme in phosphatidylcholine synthesis .
	manualset3
96046	6	400750	13	NULL	NULL	0	NULL	activity of cholinephosphate cytidylyltransferase 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second example , a relationship was established between changes in membrane lipid composition during lung development and the activity of cholinephosphate cytidylyltransferase , the rate-limiting enzyme in phosphatidylcholine synthesis .
	manualset3
96047	7	400750	13	NULL	NULL	0	NULL	rate-limiting enzyme 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second example , a relationship was established between changes in membrane lipid composition during lung development and the activity of cholinephosphate cytidylyltransferase , the rate-limiting enzyme in phosphatidylcholine synthesis .
	manualset3
96048	8	400750	13	NULL	NULL	0	NULL	phosphatidylcholine synthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second example , a relationship was established between changes in membrane lipid composition during lung development and the activity of cholinephosphate cytidylyltransferase , the rate-limiting enzyme in phosphatidylcholine synthesis .
	manualset3
96049	1	400751	13	NULL	NULL	NULL	NULL	12 of 13 liver biopsy specimens	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	12 of 13 liver biopsy specimens were also positive for antigen .
	manualset3
96050	2	400751	13	NULL	NULL	NULL	NULL	antigen	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	12 of 13 liver biopsy specimens were also positive for antigen .
	manualset3
96051	1	400752	13	NULL	NULL	0	NULL	second group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second group are 4 kindreds characterized by very low , but measurable , protein C levels in homozygotes who survived beyond the neonatal period into adulthood with histories of moderately severe thrombosis .
	manualset3
96052	2	400752	13	NULL	NULL	0	NULL	4 kindreds	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second group are 4 kindreds characterized by very low , but measurable , protein C levels in homozygotes who survived beyond the neonatal period into adulthood with histories of moderately severe thrombosis .
	manualset3
96053	3	400752	13	NULL	NULL	0	NULL	protein C levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second group are 4 kindreds characterized by very low , but measurable , protein C levels in homozygotes who survived beyond the neonatal period into adulthood with histories of moderately severe thrombosis .
	manualset3
96054	4	400752	13	NULL	NULL	0	NULL	 homozygotes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second group are 4 kindreds characterized by very low , but measurable , protein C levels in homozygotes who survived beyond the neonatal period into adulthood with histories of moderately severe thrombosis .
	manualset3
96055	5	400752	13	NULL	NULL	0	NULL	neonatal period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second group are 4 kindreds characterized by very low , but measurable , protein C levels in homozygotes who survived beyond the neonatal period into adulthood with histories of moderately severe thrombosis .
	manualset3
96056	6	400752	13	NULL	NULL	0	NULL	adulthood	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second group are 4 kindreds characterized by very low , but measurable , protein C levels in homozygotes who survived beyond the neonatal period into adulthood with histories of moderately severe thrombosis .
	manualset3
96057	7	400752	13	NULL	NULL	0	NULL	histories of moderately severe thrombosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second group are 4 kindreds characterized by very low , but measurable , protein C levels in homozygotes who survived beyond the neonatal period into adulthood with histories of moderately severe thrombosis .
	manualset3
96058	1	400753	13	NULL	NULL	0	NULL	part of the tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second one , the remaining part of the tumor was removed completely from the vertebral canal and retroperitoneal area through posterior-lateral access .
	manualset3
96059	2	400753	13	NULL	NULL	0	NULL	vertebral canal	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second one , the remaining part of the tumor was removed completely from the vertebral canal and retroperitoneal area through posterior-lateral access .
	manualset3
96060	3	400753	13	NULL	NULL	0	NULL	retroperitoneal area	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second one , the remaining part of the tumor was removed completely from the vertebral canal and retroperitoneal area through posterior-lateral access .
	manualset3
96061	4	400753	13	NULL	NULL	0	NULL	posterior-lateral access	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second one , the remaining part of the tumor was removed completely from the vertebral canal and retroperitoneal area through posterior-lateral access .
	manualset3
96062	1	400754	13	NULL	NULL	0	NULL	second part 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second part of the paper the morphological difference between the two probability density functions is used to constrain a one-dimensional , `` blind , '' iterative deconvolution at the position of an exoplanet .
	manualset3
96063	2	400754	13	NULL	NULL	0	NULL	paper 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second part of the paper the morphological difference between the two probability density functions is used to constrain a one-dimensional , `` blind , '' iterative deconvolution at the position of an exoplanet .
	manualset3
96064	3	400754	13	NULL	NULL	0	NULL	morphological difference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second part of the paper the morphological difference between the two probability density functions is used to constrain a one-dimensional , `` blind , '' iterative deconvolution at the position of an exoplanet .
	manualset3
96065	4	400754	13	NULL	NULL	0	NULL	two probability density functions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second part of the paper the morphological difference between the two probability density functions is used to constrain a one-dimensional , `` blind , '' iterative deconvolution at the position of an exoplanet .
	manualset3
96066	5	400754	13	NULL	NULL	0	NULL	deconvolution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second part of the paper the morphological difference between the two probability density functions is used to constrain a one-dimensional , `` blind , '' iterative deconvolution at the position of an exoplanet .
	manualset3
96067	6	400754	13	NULL	NULL	0	NULL	exoplanet	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second part of the paper the morphological difference between the two probability density functions is used to constrain a one-dimensional , `` blind , '' iterative deconvolution at the position of an exoplanet .
	manualset3
96068	1	400755	13	NULL	NULL	0	NULL	 second part 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second part of the study the effect of exogenous substance P ( SP ) on spontaneous as well as on nicotine-stimulated CA release was investigated .
	manualset3
96069	2	400755	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second part of the study the effect of exogenous substance P ( SP ) on spontaneous as well as on nicotine-stimulated CA release was investigated .
	manualset3
96070	3	400755	13	NULL	NULL	0	NULL	effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second part of the study the effect of exogenous substance P ( SP ) on spontaneous as well as on nicotine-stimulated CA release was investigated .
	manualset3
96071	4	400755	13	NULL	NULL	0	NULL	substance P ( SP )	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second part of the study the effect of exogenous substance P ( SP ) on spontaneous as well as on nicotine-stimulated CA release was investigated .
	manualset3
96072	5	400755	13	NULL	NULL	0	NULL	nicotine-stimulated CA release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second part of the study the effect of exogenous substance P ( SP ) on spontaneous as well as on nicotine-stimulated CA release was investigated .
	manualset3
96073	1	400756	13	NULL	NULL	0	NULL	second series	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second series , three groups of eyed eggs of Atlantic salmon allegedly differing in their innate resistance to IPNV were used ( Storset , Strand , Wetten , Kjglum & Ramstad 2007 ) .
	manualset3
96074	2	400756	13	NULL	NULL	0	NULL	 three groups	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second series , three groups of eyed eggs of Atlantic salmon allegedly differing in their innate resistance to IPNV were used ( Storset , Strand , Wetten , Kjglum & Ramstad 2007 ) .
	manualset3
96075	3	400756	13	NULL	NULL	0	NULL	eyed eggs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second series , three groups of eyed eggs of Atlantic salmon allegedly differing in their innate resistance to IPNV were used ( Storset , Strand , Wetten , Kjglum & Ramstad 2007 ) .
	manualset3
96076	4	400756	13	NULL	NULL	0	NULL	Atlantic salmon	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second series , three groups of eyed eggs of Atlantic salmon allegedly differing in their innate resistance to IPNV were used ( Storset , Strand , Wetten , Kjglum & Ramstad 2007 ) .
	manualset3
96077	5	400756	13	NULL	NULL	0	NULL	innate resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second series , three groups of eyed eggs of Atlantic salmon allegedly differing in their innate resistance to IPNV were used ( Storset , Strand , Wetten , Kjglum & Ramstad 2007 ) .
	manualset3
96078	6	400756	13	NULL	NULL	0	NULL	 IPNV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second series , three groups of eyed eggs of Atlantic salmon allegedly differing in their innate resistance to IPNV were used ( Storset , Strand , Wetten , Kjglum & Ramstad 2007 ) .
	manualset3
96079	7	400756	13	NULL	NULL	0	NULL	Storset	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second series , three groups of eyed eggs of Atlantic salmon allegedly differing in their innate resistance to IPNV were used ( Storset , Strand , Wetten , Kjglum & Ramstad 2007 ) .
	manualset3
96080	8	400756	13	NULL	NULL	0	NULL	Strand	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second series , three groups of eyed eggs of Atlantic salmon allegedly differing in their innate resistance to IPNV were used ( Storset , Strand , Wetten , Kjglum & Ramstad 2007 ) .
	manualset3
96081	9	400756	13	NULL	NULL	0	NULL	Wetten	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second series , three groups of eyed eggs of Atlantic salmon allegedly differing in their innate resistance to IPNV were used ( Storset , Strand , Wetten , Kjglum & Ramstad 2007 ) .
	manualset3
96082	10	400756	13	NULL	NULL	0	NULL	Kjglum	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second series , three groups of eyed eggs of Atlantic salmon allegedly differing in their innate resistance to IPNV were used ( Storset , Strand , Wetten , Kjglum & Ramstad 2007 ) .
	manualset3
96083	11	400756	13	NULL	NULL	0	NULL	Ramstad	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second series , three groups of eyed eggs of Atlantic salmon allegedly differing in their innate resistance to IPNV were used ( Storset , Strand , Wetten , Kjglum & Ramstad 2007 ) .
	manualset3
96084	12	400756	13	NULL	NULL	0	NULL	2007 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second series , three groups of eyed eggs of Atlantic salmon allegedly differing in their innate resistance to IPNV were used ( Storset , Strand , Wetten , Kjglum & Ramstad 2007 ) .
	manualset3
96085	1	400757	13	NULL	NULL	0	NULL	sera	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In the sera of leukemic mice soluble tumor-specific antigen could be demonstrated in the stages of early progression and regression but not in the stage of exacerbation .
	manualset3
96086	2	400757	13	NULL	NULL	0	NULL	leukemic mice soluble tumor-specific antigen	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the sera of leukemic mice soluble tumor-specific antigen could be demonstrated in the stages of early progression and regression but not in the stage of exacerbation .
	manualset3
96087	3	400757	13	NULL	NULL	NULL	NULL	 stage of early progression 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the sera of leukemic mice soluble tumor-specific antigen could be demonstrated in the stages of early progression and regression but not in the stage of exacerbation .
	manualset3
96088	4	400757	13	NULL	NULL	NULL	NULL	stage of early regression	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the sera of leukemic mice soluble tumor-specific antigen could be demonstrated in the stages of early progression and regression but not in the stage of exacerbation .
	manualset3
96090	5	400757	13	NULL	NULL	NULL	NULL	stage of exacerbation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the sera of leukemic mice soluble tumor-specific antigen could be demonstrated in the stages of early progression and regression but not in the stage of exacerbation .
	manualset3
96091	1	400758	13	NULL	NULL	0	NULL	simplest case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the simplest case of age-independent ( type 2 ) survivorship in a population of N adults , Ne = N / ( 2-T-1 ) where T is the generation time .
	manualset3
96092	2	400758	13	NULL	NULL	0	NULL	age-independent ( type 2 ) survivorship	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the simplest case of age-independent ( type 2 ) survivorship in a population of N adults , Ne = N / ( 2-T-1 ) where T is the generation time .
	manualset3
96093	3	400758	13	NULL	NULL	0	NULL	 population of N adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the simplest case of age-independent ( type 2 ) survivorship in a population of N adults , Ne = N / ( 2-T-1 ) where T is the generation time .
	manualset3
96094	4	400758	13	NULL	NULL	0	NULL	Ne = N / ( 2-T-1 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the simplest case of age-independent ( type 2 ) survivorship in a population of N adults , Ne = N / ( 2-T-1 ) where T is the generation time .
	manualset3
96095	5	400758	13	NULL	NULL	0	NULL	T is the generation time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In the simplest case of age-independent ( type 2 ) survivorship in a population of N adults , Ne = N / ( 2-T-1 ) where T is the generation time .
	manualset3
96096	1	400759	13	NULL	NULL	0	NULL	skin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the skin , several connexins are expressed and are involved in the regulation of epidermal growth and differentiation .
	manualset3
96097	2	400759	13	NULL	NULL	0	NULL	several connexins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the skin , several connexins are expressed and are involved in the regulation of epidermal growth and differentiation .
	manualset3
96098	3	400759	13	NULL	NULL	0	NULL	regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the skin , several connexins are expressed and are involved in the regulation of epidermal growth and differentiation .
	manualset3
96100	4	400759	13	NULL	NULL	0	NULL	epidermal growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the skin , several connexins are expressed and are involved in the regulation of epidermal growth and differentiation .
	manualset3
96101	5	400759	13	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the skin , several connexins are expressed and are involved in the regulation of epidermal growth and differentiation .
	manualset3
96102	1	400760	13	NULL	NULL	0	NULL	120 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	120 degrees C was seen , followed by melting of form II at 156 degrees C. At heating rates of 400 degrees C min ( -1 ) and higher , the solid-solid transition was absent and two endotherms were observed ; the form II melt at 156 degrees C and a new , lower temperature endotherm at 143 degrees C. We ascribe the transition at 143 degrees C to the melting of form III .
	manualset3
96103	2	400760	13	NULL	NULL	0	NULL	form II 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	120 degrees C was seen , followed by melting of form II at 156 degrees C. At heating rates of 400 degrees C min ( -1 ) and higher , the solid-solid transition was absent and two endotherms were observed ; the form II melt at 156 degrees C and a new , lower temperature endotherm at 143 degrees C. We ascribe the transition at 143 degrees C to the melting of form III .
	manualset3
96104	3	400760	13	NULL	NULL	0	NULL	156 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	120 degrees C was seen , followed by melting of form II at 156 degrees C. At heating rates of 400 degrees C min ( -1 ) and higher , the solid-solid transition was absent and two endotherms were observed ; the form II melt at 156 degrees C and a new , lower temperature endotherm at 143 degrees C. We ascribe the transition at 143 degrees C to the melting of form III .
	manualset3
96105	4	400760	13	NULL	NULL	0	NULL	heating rates	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	120 degrees C was seen , followed by melting of form II at 156 degrees C. At heating rates of 400 degrees C min ( -1 ) and higher , the solid-solid transition was absent and two endotherms were observed ; the form II melt at 156 degrees C and a new , lower temperature endotherm at 143 degrees C. We ascribe the transition at 143 degrees C to the melting of form III .
	manualset3
96106	5	400760	13	NULL	NULL	0	NULL	400 degrees C min ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	120 degrees C was seen , followed by melting of form II at 156 degrees C. At heating rates of 400 degrees C min ( -1 ) and higher , the solid-solid transition was absent and two endotherms were observed ; the form II melt at 156 degrees C and a new , lower temperature endotherm at 143 degrees C. We ascribe the transition at 143 degrees C to the melting of form III .
	manualset3
96107	6	400760	13	NULL	NULL	0	NULL	solid-solid transition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	120 degrees C was seen , followed by melting of form II at 156 degrees C. At heating rates of 400 degrees C min ( -1 ) and higher , the solid-solid transition was absent and two endotherms were observed ; the form II melt at 156 degrees C and a new , lower temperature endotherm at 143 degrees C. We ascribe the transition at 143 degrees C to the melting of form III .
	manualset3
96108	7	400760	13	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	120 degrees C was seen , followed by melting of form II at 156 degrees C. At heating rates of 400 degrees C min ( -1 ) and higher , the solid-solid transition was absent and two endotherms were observed ; the form II melt at 156 degrees C and a new , lower temperature endotherm at 143 degrees C. We ascribe the transition at 143 degrees C to the melting of form III .
	manualset3
96109	8	400760	13	NULL	NULL	0	NULL	endotherms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	120 degrees C was seen , followed by melting of form II at 156 degrees C. At heating rates of 400 degrees C min ( -1 ) and higher , the solid-solid transition was absent and two endotherms were observed ; the form II melt at 156 degrees C and a new , lower temperature endotherm at 143 degrees C. We ascribe the transition at 143 degrees C to the melting of form III .
	manualset3
96110	9	400760	13	NULL	NULL	0	NULL	form II	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	120 degrees C was seen , followed by melting of form II at 156 degrees C. At heating rates of 400 degrees C min ( -1 ) and higher , the solid-solid transition was absent and two endotherms were observed ; the form II melt at 156 degrees C and a new , lower temperature endotherm at 143 degrees C. We ascribe the transition at 143 degrees C to the melting of form III .
	manualset3
96111	10	400760	13	NULL	NULL	0	NULL	156 degrees C 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	120 degrees C was seen , followed by melting of form II at 156 degrees C. At heating rates of 400 degrees C min ( -1 ) and higher , the solid-solid transition was absent and two endotherms were observed ; the form II melt at 156 degrees C and a new , lower temperature endotherm at 143 degrees C. We ascribe the transition at 143 degrees C to the melting of form III .
	manualset3
96112	11	400760	13	NULL	NULL	0	NULL	lower temperature endotherm	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	120 degrees C was seen , followed by melting of form II at 156 degrees C. At heating rates of 400 degrees C min ( -1 ) and higher , the solid-solid transition was absent and two endotherms were observed ; the form II melt at 156 degrees C and a new , lower temperature endotherm at 143 degrees C. We ascribe the transition at 143 degrees C to the melting of form III .
	manualset3
96113	12	400760	13	NULL	NULL	0	NULL	143 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	120 degrees C was seen , followed by melting of form II at 156 degrees C. At heating rates of 400 degrees C min ( -1 ) and higher , the solid-solid transition was absent and two endotherms were observed ; the form II melt at 156 degrees C and a new , lower temperature endotherm at 143 degrees C. We ascribe the transition at 143 degrees C to the melting of form III .
	manualset3
96114	13	400760	13	NULL	NULL	0	NULL	transition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	120 degrees C was seen , followed by melting of form II at 156 degrees C. At heating rates of 400 degrees C min ( -1 ) and higher , the solid-solid transition was absent and two endotherms were observed ; the form II melt at 156 degrees C and a new , lower temperature endotherm at 143 degrees C. We ascribe the transition at 143 degrees C to the melting of form III .
	manualset3
96115	14	400760	13	NULL	NULL	0	NULL	143 degrees C 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	120 degrees C was seen , followed by melting of form II at 156 degrees C. At heating rates of 400 degrees C min ( -1 ) and higher , the solid-solid transition was absent and two endotherms were observed ; the form II melt at 156 degrees C and a new , lower temperature endotherm at 143 degrees C. We ascribe the transition at 143 degrees C to the melting of form III .
	manualset3
96116	15	400760	13	NULL	NULL	0	NULL	 melting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	120 degrees C was seen , followed by melting of form II at 156 degrees C. At heating rates of 400 degrees C min ( -1 ) and higher , the solid-solid transition was absent and two endotherms were observed ; the form II melt at 156 degrees C and a new , lower temperature endotherm at 143 degrees C. We ascribe the transition at 143 degrees C to the melting of form III .
	manualset3
96117	16	400760	13	NULL	NULL	0	NULL	form III	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	120 degrees C was seen , followed by melting of form II at 156 degrees C. At heating rates of 400 degrees C min ( -1 ) and higher , the solid-solid transition was absent and two endotherms were observed ; the form II melt at 156 degrees C and a new , lower temperature endotherm at 143 degrees C. We ascribe the transition at 143 degrees C to the melting of form III .
	manualset3
96118	1	400761	13	NULL	NULL	0	NULL	small intestine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the small intestine , the absorption rate constants , Ka , at pH 6.2 ranged between 0.38 h-1 for atenolol and 4.28 h-1 for penbutolol .
	manualset3
96119	2	400761	13	NULL	NULL	0	NULL	absorption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the small intestine , the absorption rate constants , Ka , at pH 6.2 ranged between 0.38 h-1 for atenolol and 4.28 h-1 for penbutolol .
	manualset3
96120	3	400761	13	NULL	NULL	0	NULL	rate constants , Ka , 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the small intestine , the absorption rate constants , Ka , at pH 6.2 ranged between 0.38 h-1 for atenolol and 4.28 h-1 for penbutolol .
	manualset3
96121	4	400761	13	NULL	NULL	0	NULL	pH 6.2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the small intestine , the absorption rate constants , Ka , at pH 6.2 ranged between 0.38 h-1 for atenolol and 4.28 h-1 for penbutolol .
	manualset3
96122	5	400761	13	NULL	NULL	0	NULL	0.38 h-1 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the small intestine , the absorption rate constants , Ka , at pH 6.2 ranged between 0.38 h-1 for atenolol and 4.28 h-1 for penbutolol .
	manualset3
96123	6	400761	13	NULL	NULL	0	NULL	 atenolol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the small intestine , the absorption rate constants , Ka , at pH 6.2 ranged between 0.38 h-1 for atenolol and 4.28 h-1 for penbutolol .
	manualset3
96124	7	400761	13	NULL	NULL	0	NULL	4.28 h-1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the small intestine , the absorption rate constants , Ka , at pH 6.2 ranged between 0.38 h-1 for atenolol and 4.28 h-1 for penbutolol .
	manualset3
96125	8	400761	13	NULL	NULL	0	NULL	penbutolol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the small intestine , the absorption rate constants , Ka , at pH 6.2 ranged between 0.38 h-1 for atenolol and 4.28 h-1 for penbutolol .
	manualset3
96126	1	400762	13	NULL	NULL	0	NULL	soleus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the soleus only 4 ( 12.3 % ) motor units remain while 10 ( 24.3 % ) remain in the EDL , showing that soleus alpha motoneurones are more sensitive to nerve injury at birth .
	manualset3
96127	2	400762	13	NULL	NULL	0	NULL	4 ( 12.3 % ) motor units	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the soleus only 4 ( 12.3 % ) motor units remain while 10 ( 24.3 % ) remain in the EDL , showing that soleus alpha motoneurones are more sensitive to nerve injury at birth .
	manualset3
96128	3	400762	13	NULL	NULL	0	NULL	10 ( 24.3 % ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the soleus only 4 ( 12.3 % ) motor units remain while 10 ( 24.3 % ) remain in the EDL , showing that soleus alpha motoneurones are more sensitive to nerve injury at birth .
	manualset3
96129	4	400762	13	NULL	NULL	0	NULL	EDL	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the soleus only 4 ( 12.3 % ) motor units remain while 10 ( 24.3 % ) remain in the EDL , showing that soleus alpha motoneurones are more sensitive to nerve injury at birth .
	manualset3
96130	5	400762	13	NULL	NULL	0	NULL	soleus alpha motoneurones	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the soleus only 4 ( 12.3 % ) motor units remain while 10 ( 24.3 % ) remain in the EDL , showing that soleus alpha motoneurones are more sensitive to nerve injury at birth .
	manualset3
96131	6	400762	13	NULL	NULL	0	NULL	nerve injury at birth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the soleus only 4 ( 12.3 % ) motor units remain while 10 ( 24.3 % ) remain in the EDL , showing that soleus alpha motoneurones are more sensitive to nerve injury at birth .
	manualset3
96132	1	400763	13	NULL	NULL	0	NULL	specimens	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In the specimens at the second-look arthroscopy , the extracellular matrix was stained more densely than at the time of fixation , especially in the middle to deep layers of the articular cartilage .
	manualset3
96133	2	400763	13	NULL	NULL	0	NULL	arthroscopy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the specimens at the second-look arthroscopy , the extracellular matrix was stained more densely than at the time of fixation , especially in the middle to deep layers of the articular cartilage .
	manualset3
96134	3	400763	13	NULL	NULL	0	NULL	extracellular matrix 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In the specimens at the second-look arthroscopy , the extracellular matrix was stained more densely than at the time of fixation , especially in the middle to deep layers of the articular cartilage .
	manualset3
96135	4	400763	13	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In the specimens at the second-look arthroscopy , the extracellular matrix was stained more densely than at the time of fixation , especially in the middle to deep layers of the articular cartilage .
	manualset3
96136	5	400763	13	NULL	NULL	0	NULL	fixation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the specimens at the second-look arthroscopy , the extracellular matrix was stained more densely than at the time of fixation , especially in the middle to deep layers of the articular cartilage .
	manualset3
96137	6	400763	13	NULL	NULL	0	NULL	middle to deep layers	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In the specimens at the second-look arthroscopy , the extracellular matrix was stained more densely than at the time of fixation , especially in the middle to deep layers of the articular cartilage .
	manualset3
96138	7	400763	13	NULL	NULL	0	NULL	articular cartilage	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In the specimens at the second-look arthroscopy , the extracellular matrix was stained more densely than at the time of fixation , especially in the middle to deep layers of the articular cartilage .
	manualset3
96139	1	400764	13	NULL	NULL	NULL	NULL	bacterial peritonitis group	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the spontaneous bacterial peritonitis group , the polymorphonuclear count was 3588 + / - 3849/microliter ( range 60-11 776 ) versus 41 + / - 138/microliter ( range 0-813 ) in the sterile group ( p less than 0.0001 ) .
	manualset3
96140	2	400764	13	NULL	NULL	0	NULL	polymorphonuclear count	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the spontaneous bacterial peritonitis group , the polymorphonuclear count was 3588 + / - 3849/microliter ( range 60-11 776 ) versus 41 + / - 138/microliter ( range 0-813 ) in the sterile group ( p less than 0.0001 ) .
	manualset3
96141	3	400764	13	NULL	NULL	0	NULL	3588 + / - 3849/microliter ( range 60-11 776 ) versus 41 + / - 138/microliter ( range 0-813 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the spontaneous bacterial peritonitis group , the polymorphonuclear count was 3588 + / - 3849/microliter ( range 60-11 776 ) versus 41 + / - 138/microliter ( range 0-813 ) in the sterile group ( p less than 0.0001 ) .
	manualset3
96142	4	400764	13	NULL	NULL	0	NULL	sterile group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the spontaneous bacterial peritonitis group , the polymorphonuclear count was 3588 + / - 3849/microliter ( range 60-11 776 ) versus 41 + / - 138/microliter ( range 0-813 ) in the sterile group ( p less than 0.0001 ) .
	manualset3
96143	5	400764	13	NULL	NULL	NULL	NULL	p less than 0.0001	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the spontaneous bacterial peritonitis group , the polymorphonuclear count was 3588 + / - 3849/microliter ( range 60-11 776 ) versus 41 + / - 138/microliter ( range 0-813 ) in the sterile group ( p less than 0.0001 ) .
	manualset3
96144	1	400765	13	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the study , membrane fouling and polarization at the membrane surface played a significant role in the formation of the strongly attached cake layer limiting membrane permeability
	manualset3
96145	2	400765	13	NULL	NULL	NULL	NULL	membrane fouling	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the study , membrane fouling and polarization at the membrane surface played a significant role in the formation of the strongly attached cake layer limiting membrane permeability
	manualset3
96146	3	400765	13	NULL	NULL	NULL	NULL	polarization	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the study , membrane fouling and polarization at the membrane surface played a significant role in the formation of the strongly attached cake layer limiting membrane permeability
	manualset3
96147	4	400765	13	NULL	NULL	0	NULL	membrane surface	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In the study , membrane fouling and polarization at the membrane surface played a significant role in the formation of the strongly attached cake layer limiting membrane permeability
	manualset3
96148	5	400765	13	NULL	NULL	0	NULL	significant role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the study , membrane fouling and polarization at the membrane surface played a significant role in the formation of the strongly attached cake layer limiting membrane permeability
	manualset3
96149	6	400765	13	NULL	NULL	0	NULL	formation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the study , membrane fouling and polarization at the membrane surface played a significant role in the formation of the strongly attached cake layer limiting membrane permeability
	manualset3
96150	7	400765	13	NULL	NULL	NULL	NULL	cake layer 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the study , membrane fouling and polarization at the membrane surface played a significant role in the formation of the strongly attached cake layer limiting membrane permeability
	manualset3
96151	8	400765	13	NULL	NULL	0	NULL	membrane permeability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the study , membrane fouling and polarization at the membrane surface played a significant role in the formation of the strongly attached cake layer limiting membrane permeability
	manualset3
96152	1	400766	13	NULL	NULL	0	NULL	subline IGROVI-C10 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the subline IGROVI-C10 , a 10-fold resistant subline of IGROVI , AmB at 10 mg/l allowed recovery to the level of sensitivity seen in the parental cell line in the absence of AmB but not to the level observed in the presence of AmB .
	manualset3
96153	2	400766	13	NULL	NULL	0	NULL	10-fold resistant subline of IGROVI	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the subline IGROVI-C10 , a 10-fold resistant subline of IGROVI , AmB at 10 mg/l allowed recovery to the level of sensitivity seen in the parental cell line in the absence of AmB but not to the level observed in the presence of AmB .
	manualset3
96154	3	400766	13	NULL	NULL	0	NULL	AmB	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the subline IGROVI-C10 , a 10-fold resistant subline of IGROVI , AmB at 10 mg/l allowed recovery to the level of sensitivity seen in the parental cell line in the absence of AmB but not to the level observed in the presence of AmB .
	manualset3
96155	4	400766	13	NULL	NULL	0	NULL	10 mg/l	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the subline IGROVI-C10 , a 10-fold resistant subline of IGROVI , AmB at 10 mg/l allowed recovery to the level of sensitivity seen in the parental cell line in the absence of AmB but not to the level observed in the presence of AmB .
	manualset3
96156	5	400766	13	NULL	NULL	0	NULL	recovery	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the subline IGROVI-C10 , a 10-fold resistant subline of IGROVI , AmB at 10 mg/l allowed recovery to the level of sensitivity seen in the parental cell line in the absence of AmB but not to the level observed in the presence of AmB .
	manualset3
96157	6	400766	13	NULL	NULL	0	NULL	 level of sensitivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the subline IGROVI-C10 , a 10-fold resistant subline of IGROVI , AmB at 10 mg/l allowed recovery to the level of sensitivity seen in the parental cell line in the absence of AmB but not to the level observed in the presence of AmB .
	manualset3
96158	7	400766	13	NULL	NULL	0	NULL	parental cell line 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the subline IGROVI-C10 , a 10-fold resistant subline of IGROVI , AmB at 10 mg/l allowed recovery to the level of sensitivity seen in the parental cell line in the absence of AmB but not to the level observed in the presence of AmB .
	manualset3
96159	8	400766	13	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the subline IGROVI-C10 , a 10-fold resistant subline of IGROVI , AmB at 10 mg/l allowed recovery to the level of sensitivity seen in the parental cell line in the absence of AmB but not to the level observed in the presence of AmB .
	manualset3
96160	9	400766	13	NULL	NULL	0	NULL	AmB 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the subline IGROVI-C10 , a 10-fold resistant subline of IGROVI , AmB at 10 mg/l allowed recovery to the level of sensitivity seen in the parental cell line in the absence of AmB but not to the level observed in the presence of AmB .
	manualset3
96161	10	400766	13	NULL	NULL	0	NULL	level	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the subline IGROVI-C10 , a 10-fold resistant subline of IGROVI , AmB at 10 mg/l allowed recovery to the level of sensitivity seen in the parental cell line in the absence of AmB but not to the level observed in the presence of AmB .
	manualset3
96162	11	400766	13	NULL	NULL	0	NULL	 presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the subline IGROVI-C10 , a 10-fold resistant subline of IGROVI , AmB at 10 mg/l allowed recovery to the level of sensitivity seen in the parental cell line in the absence of AmB but not to the level observed in the presence of AmB .
	manualset3
96163	12	400766	13	NULL	NULL	NULL	NULL	AmB	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the subline IGROVI-C10 , a 10-fold resistant subline of IGROVI , AmB at 10 mg/l allowed recovery to the level of sensitivity seen in the parental cell line in the absence of AmB but not to the level observed in the presence of AmB .
	manualset3
96164	1	400767	13	NULL	NULL	0	NULL	sulfone mol-ecule	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the sulfone mol-ecule of the title compound , C ( 12 ) H ( 12 ) N ( 2 ) O ( 2 ) SC ( 2 ) H ( 3 ) N , the two benzene rings are oriented at a dihedral angle of 80.69 ( 3 ) .
	manualset3
96165	2	400767	13	NULL	NULL	0	NULL	title compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the sulfone mol-ecule of the title compound , C ( 12 ) H ( 12 ) N ( 2 ) O ( 2 ) SC ( 2 ) H ( 3 ) N , the two benzene rings are oriented at a dihedral angle of 80.69 ( 3 ) .
	manualset3
96166	3	400767	13	NULL	NULL	0	NULL	C ( 12 ) H ( 12 ) N ( 2 ) O ( 2 ) SC ( 2 ) H ( 3 ) N	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the sulfone mol-ecule of the title compound , C ( 12 ) H ( 12 ) N ( 2 ) O ( 2 ) SC ( 2 ) H ( 3 ) N , the two benzene rings are oriented at a dihedral angle of 80.69 ( 3 ) .
	manualset3
96167	4	400767	13	NULL	NULL	0	NULL	two benzene rings	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the sulfone mol-ecule of the title compound , C ( 12 ) H ( 12 ) N ( 2 ) O ( 2 ) SC ( 2 ) H ( 3 ) N , the two benzene rings are oriented at a dihedral angle of 80.69 ( 3 ) .
	manualset3
96168	5	400767	13	NULL	NULL	0	NULL	dihedral angle of 80.69 ( 3 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the sulfone mol-ecule of the title compound , C ( 12 ) H ( 12 ) N ( 2 ) O ( 2 ) SC ( 2 ) H ( 3 ) N , the two benzene rings are oriented at a dihedral angle of 80.69 ( 3 ) .
	manualset3
96169	1	400768	13	NULL	NULL	0	NULL	tectum opticum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the tectum opticum of the adult neotenic A. mexicanum , responses of single neuronal units to diffuse illumination and moving visual stimuli have been investigated .
	manualset3
96170	2	400768	13	NULL	NULL	0	NULL	adult neotenic A. mexicanum 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the tectum opticum of the adult neotenic A. mexicanum , responses of single neuronal units to diffuse illumination and moving visual stimuli have been investigated .
	manualset3
96171	3	400768	13	NULL	NULL	0	NULL	responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the tectum opticum of the adult neotenic A. mexicanum , responses of single neuronal units to diffuse illumination and moving visual stimuli have been investigated .
	manualset3
96172	4	400768	13	NULL	NULL	0	NULL	single neuronal units	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the tectum opticum of the adult neotenic A. mexicanum , responses of single neuronal units to diffuse illumination and moving visual stimuli have been investigated .
	manualset3
96173	5	400768	13	NULL	NULL	0	NULL	 illumination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the tectum opticum of the adult neotenic A. mexicanum , responses of single neuronal units to diffuse illumination and moving visual stimuli have been investigated .
	manualset3
96174	6	400768	13	NULL	NULL	0	NULL	visual stimuli 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the tectum opticum of the adult neotenic A. mexicanum , responses of single neuronal units to diffuse illumination and moving visual stimuli have been investigated .
	manualset3
96175	1	400769	13	NULL	NULL	0	NULL	125 : 639 -649	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	125 : 639 -649 ) , ZAP-70 may be localized close to its downstream targets .
	manualset3
96176	2	400769	13	NULL	NULL	0	NULL	ZAP-70	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	125 : 639 -649 ) , ZAP-70 may be localized close to its downstream targets .
	manualset3
96177	3	400769	13	NULL	NULL	0	NULL	downstream targets 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	125 : 639 -649 ) , ZAP-70 may be localized close to its downstream targets .
	manualset3
96178	1	400770	13	NULL	NULL	0	NULL	temporalis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the temporalis and masseter muscles , early and late phases ( ES1 and ES2 ) were observed .
	manualset3
96179	2	400770	13	NULL	NULL	0	NULL	masseter muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the temporalis and masseter muscles , early and late phases ( ES1 and ES2 ) were observed .
	manualset3
96180	3	400770	13	NULL	NULL	0	NULL	early phase	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the temporalis and masseter muscles , early and late phases ( ES1 and ES2 ) were observed .
	manualset3
96181	4	400770	13	NULL	NULL	0	NULL	late phase	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the temporalis and masseter muscles , early and late phases ( ES1 and ES2 ) were observed .
	manualset3
96182	5	400770	13	NULL	NULL	0	NULL	ES1	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the temporalis and masseter muscles , early and late phases ( ES1 and ES2 ) were observed .
	manualset3
96183	6	400770	13	NULL	NULL	0	NULL	ES2	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the temporalis and masseter muscles , early and late phases ( ES1 and ES2 ) were observed .
	manualset3
96184	1	400771	13	NULL	NULL	0	NULL	 tetrapyrrole biosynthetic pathway 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the tetrapyrrole biosynthetic pathway , isoforms of glutamyl-tRNA reductase ( HEMA2 ) and ferrochelatase1 ( FC1 ) are mainly expressed in nonphotosynthetic tissues .
	manualset3
96185	2	400771	13	NULL	NULL	0	NULL	isoforms of glutamyl-tRNA reductase ( HEMA2 )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the tetrapyrrole biosynthetic pathway , isoforms of glutamyl-tRNA reductase ( HEMA2 ) and ferrochelatase1 ( FC1 ) are mainly expressed in nonphotosynthetic tissues .
	manualset3
96186	3	400771	13	NULL	NULL	0	NULL	ferrochelatase1 ( FC1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the tetrapyrrole biosynthetic pathway , isoforms of glutamyl-tRNA reductase ( HEMA2 ) and ferrochelatase1 ( FC1 ) are mainly expressed in nonphotosynthetic tissues .
	manualset3
96187	4	400771	13	NULL	NULL	0	NULL	 nonphotosynthetic tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In the tetrapyrrole biosynthetic pathway , isoforms of glutamyl-tRNA reductase ( HEMA2 ) and ferrochelatase1 ( FC1 ) are mainly expressed in nonphotosynthetic tissues .
	manualset3
96188	1	400772	13	NULL	NULL	0	NULL	third experiment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the third experiment , 2 of the 3 control calves developed moderate to severe consolidation , but P. hemolytica was isolated only from one of them .
	manualset3
96189	2	400772	13	NULL	NULL	0	NULL	2 of the 3	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the third experiment , 2 of the 3 control calves developed moderate to severe consolidation , but P. hemolytica was isolated only from one of them .
	manualset3
96190	3	400772	13	NULL	NULL	0	NULL	control calves	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the third experiment , 2 of the 3 control calves developed moderate to severe consolidation , but P. hemolytica was isolated only from one of them .
	manualset3
96191	4	400772	13	NULL	NULL	0	NULL	moderate to severe consolidation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the third experiment , 2 of the 3 control calves developed moderate to severe consolidation , but P. hemolytica was isolated only from one of them .
	manualset3
96192	5	400772	13	NULL	NULL	0	NULL	P. hemolytica 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the third experiment , 2 of the 3 control calves developed moderate to severe consolidation , but P. hemolytica was isolated only from one of them .
	manualset3
96193	1	400773	13	NULL	NULL	0	NULL	title compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , ( Cu ( 2 ) ( C ( 8 ) H ( 11 ) N ( 2 ) O ( 3 ) S ) ( 2 ) Cl ( 2 ) ) , the Cu atoms are five-coordinated in a distorted square-pyramidal geometry by three donor atoms of the deprotonated anionic 2 - ( 2-pyridylmethyl-amino ) ethanesulfonate ( pmt ) ligand and two Cl atoms .
	manualset3
96194	2	400773	13	NULL	NULL	0	NULL	( Cu ( 2 ) ( C ( 8 ) H ( 11 ) N ( 2 ) O ( 3 ) S ) ( 2 ) Cl ( 2 ) ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , ( Cu ( 2 ) ( C ( 8 ) H ( 11 ) N ( 2 ) O ( 3 ) S ) ( 2 ) Cl ( 2 ) ) , the Cu atoms are five-coordinated in a distorted square-pyramidal geometry by three donor atoms of the deprotonated anionic 2 - ( 2-pyridylmethyl-amino ) ethanesulfonate ( pmt ) ligand and two Cl atoms .
	manualset3
96195	3	400773	13	NULL	NULL	0	NULL	Cu atoms	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , ( Cu ( 2 ) ( C ( 8 ) H ( 11 ) N ( 2 ) O ( 3 ) S ) ( 2 ) Cl ( 2 ) ) , the Cu atoms are five-coordinated in a distorted square-pyramidal geometry by three donor atoms of the deprotonated anionic 2 - ( 2-pyridylmethyl-amino ) ethanesulfonate ( pmt ) ligand and two Cl atoms .
	manualset3
96196	4	400773	13	NULL	NULL	NULL	NULL	square-pyramidal geometry	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the title compound , ( Cu ( 2 ) ( C ( 8 ) H ( 11 ) N ( 2 ) O ( 3 ) S ) ( 2 ) Cl ( 2 ) ) , the Cu atoms are five-coordinated in a distorted square-pyramidal geometry by three donor atoms of the deprotonated anionic 2 - ( 2-pyridylmethyl-amino ) ethanesulfonate ( pmt ) ligand and two Cl atoms .
	manualset3
96197	5	400773	13	NULL	NULL	0	NULL	 three donor atoms	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , ( Cu ( 2 ) ( C ( 8 ) H ( 11 ) N ( 2 ) O ( 3 ) S ) ( 2 ) Cl ( 2 ) ) , the Cu atoms are five-coordinated in a distorted square-pyramidal geometry by three donor atoms of the deprotonated anionic 2 - ( 2-pyridylmethyl-amino ) ethanesulfonate ( pmt ) ligand and two Cl atoms .
	manualset3
96198	6	400773	13	NULL	NULL	0	NULL	anionic 2 - ( 2-pyridylmethyl-amino ) ethanesulfonate ( pmt ) ligand 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , ( Cu ( 2 ) ( C ( 8 ) H ( 11 ) N ( 2 ) O ( 3 ) S ) ( 2 ) Cl ( 2 ) ) , the Cu atoms are five-coordinated in a distorted square-pyramidal geometry by three donor atoms of the deprotonated anionic 2 - ( 2-pyridylmethyl-amino ) ethanesulfonate ( pmt ) ligand and two Cl atoms .
	manualset3
96199	7	400773	13	NULL	NULL	0	NULL	two Cl atoms 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , ( Cu ( 2 ) ( C ( 8 ) H ( 11 ) N ( 2 ) O ( 3 ) S ) ( 2 ) Cl ( 2 ) ) , the Cu atoms are five-coordinated in a distorted square-pyramidal geometry by three donor atoms of the deprotonated anionic 2 - ( 2-pyridylmethyl-amino ) ethanesulfonate ( pmt ) ligand and two Cl atoms .
	manualset3
96200	1	400774	13	NULL	NULL	0	NULL	title compound 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , ( Y ( 2 ) ( C ( 4 ) H ( 4 ) O ( 4 ) ) ( 2 ) ( C ( 2 ) O ( 4 ) ) ( H ( 2 ) O ) ( 2 ) ) ( n ) , the flexible succinate anion assumes a gauche conformation and bridges the eight-coordinated Y atoms , generating two-dimensional layers parallel to ( 010 ) .
	manualset3
96201	2	400774	13	NULL	NULL	0	NULL	( Y ( 2 ) ( C ( 4 ) H ( 4 ) O ( 4 ) ) ( 2 ) ( C ( 2 ) O ( 4 ) ) ( H ( 2 ) O ) ( 2 ) ) ( n ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , ( Y ( 2 ) ( C ( 4 ) H ( 4 ) O ( 4 ) ) ( 2 ) ( C ( 2 ) O ( 4 ) ) ( H ( 2 ) O ) ( 2 ) ) ( n ) , the flexible succinate anion assumes a gauche conformation and bridges the eight-coordinated Y atoms , generating two-dimensional layers parallel to ( 010 ) .
	manualset3
96202	3	400774	13	NULL	NULL	0	NULL	succinate anion	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , ( Y ( 2 ) ( C ( 4 ) H ( 4 ) O ( 4 ) ) ( 2 ) ( C ( 2 ) O ( 4 ) ) ( H ( 2 ) O ) ( 2 ) ) ( n ) , the flexible succinate anion assumes a gauche conformation and bridges the eight-coordinated Y atoms , generating two-dimensional layers parallel to ( 010 ) .
	manualset3
96203	4	400774	13	NULL	NULL	NULL	NULL	gauche conformation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the title compound , ( Y ( 2 ) ( C ( 4 ) H ( 4 ) O ( 4 ) ) ( 2 ) ( C ( 2 ) O ( 4 ) ) ( H ( 2 ) O ) ( 2 ) ) ( n ) , the flexible succinate anion assumes a gauche conformation and bridges the eight-coordinated Y atoms , generating two-dimensional layers parallel to ( 010 ) .
	manualset3
96204	5	400774	13	NULL	NULL	0	NULL	coordinated Y atoms 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , ( Y ( 2 ) ( C ( 4 ) H ( 4 ) O ( 4 ) ) ( 2 ) ( C ( 2 ) O ( 4 ) ) ( H ( 2 ) O ) ( 2 ) ) ( n ) , the flexible succinate anion assumes a gauche conformation and bridges the eight-coordinated Y atoms , generating two-dimensional layers parallel to ( 010 ) .
	manualset3
96205	6	400774	13	NULL	NULL	0	NULL	 two-dimensional layers parallel to ( 010 ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , ( Y ( 2 ) ( C ( 4 ) H ( 4 ) O ( 4 ) ) ( 2 ) ( C ( 2 ) O ( 4 ) ) ( H ( 2 ) O ) ( 2 ) ) ( n ) , the flexible succinate anion assumes a gauche conformation and bridges the eight-coordinated Y atoms , generating two-dimensional layers parallel to ( 010 ) .
	manualset3
96206	1	400775	13	NULL	NULL	0	NULL	title compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , C ( 15 ) H ( 14 ) ClNO , the ortho - and meta-methyl substituents in the aniline ring are anti to the N-H bond .
	manualset3
96207	2	400775	13	NULL	NULL	0	NULL	C ( 15 ) H ( 14 ) ClNO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , C ( 15 ) H ( 14 ) ClNO , the ortho - and meta-methyl substituents in the aniline ring are anti to the N-H bond .
	manualset3
96208	3	400775	13	NULL	NULL	0	NULL	ortho-methyl substituents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , C ( 15 ) H ( 14 ) ClNO , the ortho - and meta-methyl substituents in the aniline ring are anti to the N-H bond .
	manualset3
96209	4	400775	13	NULL	NULL	0	NULL	meta-methyl substituents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , C ( 15 ) H ( 14 ) ClNO , the ortho - and meta-methyl substituents in the aniline ring are anti to the N-H bond .
	manualset3
96210	5	400775	13	NULL	NULL	0	NULL	 aniline ring 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , C ( 15 ) H ( 14 ) ClNO , the ortho - and meta-methyl substituents in the aniline ring are anti to the N-H bond .
	manualset3
96211	6	400775	13	NULL	NULL	0	NULL	 N-H bond	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , C ( 15 ) H ( 14 ) ClNO , the ortho - and meta-methyl substituents in the aniline ring are anti to the N-H bond .
	manualset3
96212	1	400776	13	NULL	NULL	0	NULL	 title compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , C ( 18 ) H ( 15 ) Cl ( 2 ) N ( 3 ) O ( 2 ) Se , the selenadiazole ring makes dihedral angles of 49.87 ( 3 ) and 55.70 ( 3 ) with the two benzene rings .
	manualset3
96213	2	400776	13	NULL	NULL	0	NULL	C ( 18 ) H ( 15 ) Cl ( 2 ) N ( 3 ) O ( 2 ) Se	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , C ( 18 ) H ( 15 ) Cl ( 2 ) N ( 3 ) O ( 2 ) Se , the selenadiazole ring makes dihedral angles of 49.87 ( 3 ) and 55.70 ( 3 ) with the two benzene rings .
	manualset3
96214	3	400776	13	NULL	NULL	0	NULL	selenadiazole ring	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , C ( 18 ) H ( 15 ) Cl ( 2 ) N ( 3 ) O ( 2 ) Se , the selenadiazole ring makes dihedral angles of 49.87 ( 3 ) and 55.70 ( 3 ) with the two benzene rings .
	manualset3
96215	4	400776	13	NULL	NULL	0	NULL	 dihedral angles of 49.87 ( 3 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , C ( 18 ) H ( 15 ) Cl ( 2 ) N ( 3 ) O ( 2 ) Se , the selenadiazole ring makes dihedral angles of 49.87 ( 3 ) and 55.70 ( 3 ) with the two benzene rings .
	manualset3
96216	5	400776	13	NULL	NULL	0	NULL	dihedral angles of  55.70 ( 3 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , C ( 18 ) H ( 15 ) Cl ( 2 ) N ( 3 ) O ( 2 ) Se , the selenadiazole ring makes dihedral angles of 49.87 ( 3 ) and 55.70 ( 3 ) with the two benzene rings .
	manualset3
96217	6	400776	13	NULL	NULL	0	NULL	two benzene rings	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , C ( 18 ) H ( 15 ) Cl ( 2 ) N ( 3 ) O ( 2 ) Se , the selenadiazole ring makes dihedral angles of 49.87 ( 3 ) and 55.70 ( 3 ) with the two benzene rings .
	manualset3
96218	1	400777	13	NULL	NULL	0	NULL	title compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , C ( 21 ) H ( 21 ) ClN ( 2 ) O ( 2 ) , the dihydro-isoxazole ring adopts an envelope conformation and the piperidinone ring is in a chair conformation .
	manualset3
96219	2	400777	13	NULL	NULL	0	NULL	C ( 21 ) H ( 21 ) ClN ( 2 ) O ( 2 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , C ( 21 ) H ( 21 ) ClN ( 2 ) O ( 2 ) , the dihydro-isoxazole ring adopts an envelope conformation and the piperidinone ring is in a chair conformation .
	manualset3
96220	3	400777	13	NULL	NULL	0	NULL	dihydro-isoxazole ring	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , C ( 21 ) H ( 21 ) ClN ( 2 ) O ( 2 ) , the dihydro-isoxazole ring adopts an envelope conformation and the piperidinone ring is in a chair conformation .
	manualset3
96221	4	400777	13	NULL	NULL	0	NULL	envelope conformation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , C ( 21 ) H ( 21 ) ClN ( 2 ) O ( 2 ) , the dihydro-isoxazole ring adopts an envelope conformation and the piperidinone ring is in a chair conformation .
	manualset3
96222	5	400777	13	NULL	NULL	0	NULL	piperidinone ring 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , C ( 21 ) H ( 21 ) ClN ( 2 ) O ( 2 ) , the dihydro-isoxazole ring adopts an envelope conformation and the piperidinone ring is in a chair conformation .
	manualset3
96223	6	400777	13	NULL	NULL	0	NULL	chair conformation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , C ( 21 ) H ( 21 ) ClN ( 2 ) O ( 2 ) , the dihydro-isoxazole ring adopts an envelope conformation and the piperidinone ring is in a chair conformation .
	manualset3
96224	1	400778	13	NULL	NULL	0	NULL	 title compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , C ( 21 ) H ( 21 ) N ( 3 ) O ( 3 ) , the relative stereochemistry of the four stereogenic C atoms has been determined .
	manualset3
96225	2	400778	13	NULL	NULL	0	NULL	C ( 21 ) H ( 21 ) N ( 3 ) O ( 3 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , C ( 21 ) H ( 21 ) N ( 3 ) O ( 3 ) , the relative stereochemistry of the four stereogenic C atoms has been determined .
	manualset3
96226	3	400778	13	NULL	NULL	0	NULL	stereochemistry	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , C ( 21 ) H ( 21 ) N ( 3 ) O ( 3 ) , the relative stereochemistry of the four stereogenic C atoms has been determined .
	manualset3
96227	4	400778	13	NULL	NULL	0	NULL	four stereogenic C atoms	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , C ( 21 ) H ( 21 ) N ( 3 ) O ( 3 ) , the relative stereochemistry of the four stereogenic C atoms has been determined .
	manualset3
96228	1	400779	13	NULL	NULL	0	NULL	title compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , C ( 31 ) H ( 29 ) ClN ( 2 ) O ( 2 ) S , the pyrrolidine ring adopts an envelope conformation with the methine C atom adjacent to the NH group as the flap atom .
	manualset3
96229	2	400779	13	NULL	NULL	0	NULL	C ( 31 ) H ( 29 ) ClN ( 2 ) O ( 2 ) S 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , C ( 31 ) H ( 29 ) ClN ( 2 ) O ( 2 ) S , the pyrrolidine ring adopts an envelope conformation with the methine C atom adjacent to the NH group as the flap atom .
	manualset3
96230	3	400779	13	NULL	NULL	0	NULL	pyrrolidine ring 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , C ( 31 ) H ( 29 ) ClN ( 2 ) O ( 2 ) S , the pyrrolidine ring adopts an envelope conformation with the methine C atom adjacent to the NH group as the flap atom .
	manualset3
96231	4	400779	13	NULL	NULL	0	NULL	envelope conformation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , C ( 31 ) H ( 29 ) ClN ( 2 ) O ( 2 ) S , the pyrrolidine ring adopts an envelope conformation with the methine C atom adjacent to the NH group as the flap atom .
	manualset3
96232	5	400779	13	NULL	NULL	0	NULL	methine C atom	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , C ( 31 ) H ( 29 ) ClN ( 2 ) O ( 2 ) S , the pyrrolidine ring adopts an envelope conformation with the methine C atom adjacent to the NH group as the flap atom .
	manualset3
96233	6	400779	13	NULL	NULL	0	NULL	NH group	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , C ( 31 ) H ( 29 ) ClN ( 2 ) O ( 2 ) S , the pyrrolidine ring adopts an envelope conformation with the methine C atom adjacent to the NH group as the flap atom .
	manualset3
96234	7	400779	13	NULL	NULL	0	NULL	flap atom 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	In the title compound , C ( 31 ) H ( 29 ) ClN ( 2 ) O ( 2 ) S , the pyrrolidine ring adopts an envelope conformation with the methine C atom adjacent to the NH group as the flap atom .
	manualset3
96235	1	400780	13	NULL	NULL	0	NULL	125I-Antisauvagine-30 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	125I-Antisauvagine-30 : a novel and specific high-affinity radioligand for the characterization of corticotropin-releasing factor type 2 receptors .
	manualset3
96236	2	400780	13	NULL	NULL	0	NULL	novel and specific high-affinity radioligand	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	125I-Antisauvagine-30 : a novel and specific high-affinity radioligand for the characterization of corticotropin-releasing factor type 2 receptors .
	manualset3
96237	3	400780	13	NULL	NULL	0	NULL	characterization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	125I-Antisauvagine-30 : a novel and specific high-affinity radioligand for the characterization of corticotropin-releasing factor type 2 receptors .
	manualset3
96238	4	400780	13	NULL	NULL	0	NULL	corticotropin-releasing factor type 2 receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	125I-Antisauvagine-30 : a novel and specific high-affinity radioligand for the characterization of corticotropin-releasing factor type 2 receptors .
	manualset3
96239	1	400781	13	NULL	NULL	0	NULL	transformants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the transformants the amount of Rubisco protein was not reduced , but both activation state and carboxylation efficiency of photosynthesis were lowered .
	manualset3
96240	2	400781	13	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the transformants the amount of Rubisco protein was not reduced , but both activation state and carboxylation efficiency of photosynthesis were lowered .
	manualset3
96241	3	400781	13	NULL	NULL	0	NULL	 Rubisco protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the transformants the amount of Rubisco protein was not reduced , but both activation state and carboxylation efficiency of photosynthesis were lowered .
	manualset3
96242	4	400781	13	NULL	NULL	0	NULL	activation state	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the transformants the amount of Rubisco protein was not reduced , but both activation state and carboxylation efficiency of photosynthesis were lowered .
	manualset3
96243	5	400781	13	NULL	NULL	0	NULL	carboxylation efficiency 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the transformants the amount of Rubisco protein was not reduced , but both activation state and carboxylation efficiency of photosynthesis were lowered .
	manualset3
96244	6	400781	13	NULL	NULL	0	NULL	photosynthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the transformants the amount of Rubisco protein was not reduced , but both activation state and carboxylation efficiency of photosynthesis were lowered .
	manualset3
96245	1	400782	13	NULL	NULL	0	NULL	tropics	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the tropics , the botfly Dermatobia hominis and the NWS Cochliomyia hominivorax are the most important myiasis agents in cattle .
	manualset3
96246	2	400782	13	NULL	NULL	0	NULL	botfly Dermatobia hominis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the tropics , the botfly Dermatobia hominis and the NWS Cochliomyia hominivorax are the most important myiasis agents in cattle .
	manualset3
96247	3	400782	13	NULL	NULL	0	NULL	NWS Cochliomyia hominivorax	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the tropics , the botfly Dermatobia hominis and the NWS Cochliomyia hominivorax are the most important myiasis agents in cattle .
	manualset3
96248	4	400782	13	NULL	NULL	0	NULL	myiasis agents 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the tropics , the botfly Dermatobia hominis and the NWS Cochliomyia hominivorax are the most important myiasis agents in cattle .
	manualset3
96249	5	400782	13	NULL	NULL	0	NULL	cattle	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the tropics , the botfly Dermatobia hominis and the NWS Cochliomyia hominivorax are the most important myiasis agents in cattle .
	manualset3
96250	1	400783	13	NULL	NULL	0	NULL	two Sna - mutants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the two Sna - mutants and one Ndv mutant , Tn5 had inserted into plasmid pCFN42d outside the region of nif homology .
	manualset3
96251	2	400783	13	NULL	NULL	0	NULL	one Ndv mutant	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the two Sna - mutants and one Ndv mutant , Tn5 had inserted into plasmid pCFN42d outside the region of nif homology .
	manualset3
96252	3	400783	13	NULL	NULL	NULL	NULL	Tn5	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the two Sna - mutants and one Ndv mutant , Tn5 had inserted into plasmid pCFN42d outside the region of nif homology .
	manualset3
96253	4	400783	13	NULL	NULL	NULL	NULL	plasmid pCFN42d	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the two Sna - mutants and one Ndv mutant , Tn5 had inserted into plasmid pCFN42d outside the region of nif homology .
	manualset3
96254	5	400783	13	NULL	NULL	0	NULL	region of nif homology	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the two Sna - mutants and one Ndv mutant , Tn5 had inserted into plasmid pCFN42d outside the region of nif homology .
	manualset3
96255	1	400784	13	NULL	NULL	0	NULL	 two larval stages	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the two larval stages the most extensive pattern of IR was observed with anti-FMRFamide and anti-CARP .
	manualset3
96256	2	400784	13	NULL	NULL	0	NULL	extensive pattern of IR	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the two larval stages the most extensive pattern of IR was observed with anti-FMRFamide and anti-CARP .
	manualset3
96257	3	400784	13	NULL	NULL	0	NULL	anti-FMRFamide	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the two larval stages the most extensive pattern of IR was observed with anti-FMRFamide and anti-CARP .
	manualset3
96259	4	400784	13	NULL	NULL	0	NULL	anti-CARP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the two larval stages the most extensive pattern of IR was observed with anti-FMRFamide and anti-CARP .
	manualset3
96260	1	400785	13	NULL	NULL	0	NULL	gland	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the unoperated gland , isoprenaline caused depolarizations which were slowly developing , long-lasting and of low amplitude .
	manualset3
96261	2	400785	13	NULL	NULL	0	NULL	isoprenaline	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the unoperated gland , isoprenaline caused depolarizations which were slowly developing , long-lasting and of low amplitude .
	manualset3
96262	3	400785	13	NULL	NULL	0	NULL	depolarizations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the unoperated gland , isoprenaline caused depolarizations which were slowly developing , long-lasting and of low amplitude .
	manualset3
96263	4	400785	13	NULL	NULL	0	NULL	 low amplitude 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the unoperated gland , isoprenaline caused depolarizations which were slowly developing , long-lasting and of low amplitude .
	manualset3
96264	1	400786	13	NULL	NULL	0	NULL	wild-type mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the wild-type mice , ANP exhibited higher potency in the veins than in the arteries ( EC ( 50 ) values wild-type mice : artery , 8 + / - 3 x 10 ( -9 ) M , n = 5 vs. vein , 6 + / - 4 x 10 ( -10 ) M , n = 5 ; P & lt ; 0.05 ) .
	manualset3
96265	2	400786	13	NULL	NULL	0	NULL	ANP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the wild-type mice , ANP exhibited higher potency in the veins than in the arteries ( EC ( 50 ) values wild-type mice : artery , 8 + / - 3 x 10 ( -9 ) M , n = 5 vs. vein , 6 + / - 4 x 10 ( -10 ) M , n = 5 ; P & lt ; 0.05 ) .
	manualset3
96266	3	400786	13	NULL	NULL	0	NULL	higher potency 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the wild-type mice , ANP exhibited higher potency in the veins than in the arteries ( EC ( 50 ) values wild-type mice : artery , 8 + / - 3 x 10 ( -9 ) M , n = 5 vs. vein , 6 + / - 4 x 10 ( -10 ) M , n = 5 ; P & lt ; 0.05 ) .
	manualset3
96267	4	400786	13	NULL	NULL	0	NULL	veins	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the wild-type mice , ANP exhibited higher potency in the veins than in the arteries ( EC ( 50 ) values wild-type mice : artery , 8 + / - 3 x 10 ( -9 ) M , n = 5 vs. vein , 6 + / - 4 x 10 ( -10 ) M , n = 5 ; P & lt ; 0.05 ) .
	manualset3
96268	5	400786	13	NULL	NULL	0	NULL	arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the wild-type mice , ANP exhibited higher potency in the veins than in the arteries ( EC ( 50 ) values wild-type mice : artery , 8 + / - 3 x 10 ( -9 ) M , n = 5 vs. vein , 6 + / - 4 x 10 ( -10 ) M , n = 5 ; P & lt ; 0.05 ) .
	manualset3
96269	6	400786	13	NULL	NULL	0	NULL	( EC ( 50 ) values 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the wild-type mice , ANP exhibited higher potency in the veins than in the arteries ( EC ( 50 ) values wild-type mice : artery , 8 + / - 3 x 10 ( -9 ) M , n = 5 vs. vein , 6 + / - 4 x 10 ( -10 ) M , n = 5 ; P & lt ; 0.05 ) .
	manualset3
96270	7	400786	13	NULL	NULL	0	NULL	wild-type mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the wild-type mice , ANP exhibited higher potency in the veins than in the arteries ( EC ( 50 ) values wild-type mice : artery , 8 + / - 3 x 10 ( -9 ) M , n = 5 vs. vein , 6 + / - 4 x 10 ( -10 ) M , n = 5 ; P & lt ; 0.05 ) .
	manualset3
96271	8	400786	13	NULL	NULL	0	NULL	 artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the wild-type mice , ANP exhibited higher potency in the veins than in the arteries ( EC ( 50 ) values wild-type mice : artery , 8 + / - 3 x 10 ( -9 ) M , n = 5 vs. vein , 6 + / - 4 x 10 ( -10 ) M , n = 5 ; P & lt ; 0.05 ) .
	manualset3
96272	9	400786	13	NULL	NULL	0	NULL	8 + / - 3 x 10 ( -9 ) M , n = 5 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the wild-type mice , ANP exhibited higher potency in the veins than in the arteries ( EC ( 50 ) values wild-type mice : artery , 8 + / - 3 x 10 ( -9 ) M , n = 5 vs. vein , 6 + / - 4 x 10 ( -10 ) M , n = 5 ; P & lt ; 0.05 ) .
	manualset3
96273	10	400786	13	NULL	NULL	0	NULL	vein	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the wild-type mice , ANP exhibited higher potency in the veins than in the arteries ( EC ( 50 ) values wild-type mice : artery , 8 + / - 3 x 10 ( -9 ) M , n = 5 vs. vein , 6 + / - 4 x 10 ( -10 ) M , n = 5 ; P & lt ; 0.05 ) .
	manualset3
96274	11	400786	13	NULL	NULL	0	NULL	6 + / - 4 x 10 ( -10 ) M , n = 5 ; P & lt ; 0.05 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the wild-type mice , ANP exhibited higher potency in the veins than in the arteries ( EC ( 50 ) values wild-type mice : artery , 8 + / - 3 x 10 ( -9 ) M , n = 5 vs. vein , 6 + / - 4 x 10 ( -10 ) M , n = 5 ; P & lt ; 0.05 ) .
	manualset3
96275	1	400787	13	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the women with residual adhesive disease in both or the only remaining adnexa after SLL , there were no pregnancies ; whereas 67 % of the women with at least one adnexa free of disease became pregnant ( P = 0.005 ) .
	manualset3
96276	2	400787	13	NULL	NULL	0	NULL	residual adhesive disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In the women with residual adhesive disease in both or the only remaining adnexa after SLL , there were no pregnancies ; whereas 67 % of the women with at least one adnexa free of disease became pregnant ( P = 0.005 ) .
	manualset3
96277	3	400787	13	NULL	NULL	0	NULL	adnexa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the women with residual adhesive disease in both or the only remaining adnexa after SLL , there were no pregnancies ; whereas 67 % of the women with at least one adnexa free of disease became pregnant ( P = 0.005 ) .
	manualset3
96278	4	400787	13	NULL	NULL	0	NULL	SLL	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the women with residual adhesive disease in both or the only remaining adnexa after SLL , there were no pregnancies ; whereas 67 % of the women with at least one adnexa free of disease became pregnant ( P = 0.005 ) .
	manualset3
96279	5	400787	13	NULL	NULL	0	NULL	pregnancies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the women with residual adhesive disease in both or the only remaining adnexa after SLL , there were no pregnancies ; whereas 67 % of the women with at least one adnexa free of disease became pregnant ( P = 0.005 ) .
	manualset3
96280	6	400787	13	NULL	NULL	0	NULL	67 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the women with residual adhesive disease in both or the only remaining adnexa after SLL , there were no pregnancies ; whereas 67 % of the women with at least one adnexa free of disease became pregnant ( P = 0.005 ) .
	manualset3
96281	7	400787	13	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the women with residual adhesive disease in both or the only remaining adnexa after SLL , there were no pregnancies ; whereas 67 % of the women with at least one adnexa free of disease became pregnant ( P = 0.005 ) .
	manualset3
96282	8	400787	13	NULL	NULL	0	NULL	one 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the women with residual adhesive disease in both or the only remaining adnexa after SLL , there were no pregnancies ; whereas 67 % of the women with at least one adnexa free of disease became pregnant ( P = 0.005 ) .
	manualset3
96283	9	400787	13	NULL	NULL	0	NULL	adnexa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the women with residual adhesive disease in both or the only remaining adnexa after SLL , there were no pregnancies ; whereas 67 % of the women with at least one adnexa free of disease became pregnant ( P = 0.005 ) .
	manualset3
96284	10	400787	13	NULL	NULL	0	NULL	disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In the women with residual adhesive disease in both or the only remaining adnexa after SLL , there were no pregnancies ; whereas 67 % of the women with at least one adnexa free of disease became pregnant ( P = 0.005 ) .
	manualset3
96286	12	400787	13	NULL	NULL	0	NULL	P = 0.005 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the women with residual adhesive disease in both or the only remaining adnexa after SLL , there were no pregnancies ; whereas 67 % of the women with at least one adnexa free of disease became pregnant ( P = 0.005 ) .
	manualset3
96287	1	400788	13	NULL	NULL	0	NULL	work 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the work presented here , we assess the relative contributions of these two mutations to the SVLM21 phenotype using site-directed mutagenesis to obtain virus encoding only the change to Leu at residue 87 of nsP1 ( SVMS319 ) , or only the change to Cys at residue 88 ( SVMS321 ) .
	manualset3
96288	2	400788	13	NULL	NULL	0	NULL	contributions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the work presented here , we assess the relative contributions of these two mutations to the SVLM21 phenotype using site-directed mutagenesis to obtain virus encoding only the change to Leu at residue 87 of nsP1 ( SVMS319 ) , or only the change to Cys at residue 88 ( SVMS321 ) .
	manualset3
96289	3	400788	13	NULL	NULL	0	NULL	two mutations to the SVLM21 phenotype	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the work presented here , we assess the relative contributions of these two mutations to the SVLM21 phenotype using site-directed mutagenesis to obtain virus encoding only the change to Leu at residue 87 of nsP1 ( SVMS319 ) , or only the change to Cys at residue 88 ( SVMS321 ) .
	manualset3
96290	4	400788	13	NULL	NULL	0	NULL	site-directed mutagenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the work presented here , we assess the relative contributions of these two mutations to the SVLM21 phenotype using site-directed mutagenesis to obtain virus encoding only the change to Leu at residue 87 of nsP1 ( SVMS319 ) , or only the change to Cys at residue 88 ( SVMS321 ) .
	manualset3
96291	5	400788	13	NULL	NULL	0	NULL	virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the work presented here , we assess the relative contributions of these two mutations to the SVLM21 phenotype using site-directed mutagenesis to obtain virus encoding only the change to Leu at residue 87 of nsP1 ( SVMS319 ) , or only the change to Cys at residue 88 ( SVMS321 ) .
	manualset3
96292	6	400788	13	NULL	NULL	0	NULL	change	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the work presented here , we assess the relative contributions of these two mutations to the SVLM21 phenotype using site-directed mutagenesis to obtain virus encoding only the change to Leu at residue 87 of nsP1 ( SVMS319 ) , or only the change to Cys at residue 88 ( SVMS321 ) .
	manualset3
96293	7	400788	13	NULL	NULL	0	NULL	Leu at residue 87	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the work presented here , we assess the relative contributions of these two mutations to the SVLM21 phenotype using site-directed mutagenesis to obtain virus encoding only the change to Leu at residue 87 of nsP1 ( SVMS319 ) , or only the change to Cys at residue 88 ( SVMS321 ) .
	manualset3
96294	8	400788	13	NULL	NULL	NULL	NULL	nsP1 ( SVMS319 )	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the work presented here , we assess the relative contributions of these two mutations to the SVLM21 phenotype using site-directed mutagenesis to obtain virus encoding only the change to Leu at residue 87 of nsP1 ( SVMS319 ) , or only the change to Cys at residue 88 ( SVMS321 ) .
	manualset3
96295	9	400788	13	NULL	NULL	0	NULL	change	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the work presented here , we assess the relative contributions of these two mutations to the SVLM21 phenotype using site-directed mutagenesis to obtain virus encoding only the change to Leu at residue 87 of nsP1 ( SVMS319 ) , or only the change to Cys at residue 88 ( SVMS321 ) .
	manualset3
96296	10	400788	13	NULL	NULL	0	NULL	Cys at residue 88 ( SVMS321 )	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In the work presented here , we assess the relative contributions of these two mutations to the SVLM21 phenotype using site-directed mutagenesis to obtain virus encoding only the change to Leu at residue 87 of nsP1 ( SVMS319 ) , or only the change to Cys at residue 88 ( SVMS321 ) .
	manualset3
96297	1	400789	13	NULL	NULL	0	NULL	 quiescent state 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In their quiescent state they serve as a storage site for vitamin A. In fibrotic liver they become activated , proliferate and they undergo transdifferentiation into myofibroblast-like cells .
	manualset3
96298	2	400789	13	NULL	NULL	0	NULL	storage site	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In their quiescent state they serve as a storage site for vitamin A. In fibrotic liver they become activated , proliferate and they undergo transdifferentiation into myofibroblast-like cells .
	manualset3
96299	3	400789	13	NULL	NULL	0	NULL	vitamin A	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In their quiescent state they serve as a storage site for vitamin A. In fibrotic liver they become activated , proliferate and they undergo transdifferentiation into myofibroblast-like cells .
	manualset3
96300	4	400789	13	NULL	NULL	0	NULL	fibrotic liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In their quiescent state they serve as a storage site for vitamin A. In fibrotic liver they become activated , proliferate and they undergo transdifferentiation into myofibroblast-like cells .
	manualset3
96301	5	400789	13	NULL	NULL	0	NULL	transdifferentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In their quiescent state they serve as a storage site for vitamin A. In fibrotic liver they become activated , proliferate and they undergo transdifferentiation into myofibroblast-like cells .
	manualset3
96302	6	400789	13	NULL	NULL	0	NULL	myofibroblast-like cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In their quiescent state they serve as a storage site for vitamin A. In fibrotic liver they become activated , proliferate and they undergo transdifferentiation into myofibroblast-like cells .
	manualset3
96303	1	400790	13	NULL	NULL	0	NULL	125I-BoNT type B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	125I-BoNT type B , applied in vitro to the murine neuromuscular junction , interacts likewise with the motor nerve terminal except that a lower proportion of internalized radioactivity is seen .
	manualset3
96304	2	400790	13	NULL	NULL	0	NULL	murine neuromuscular junction	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	125I-BoNT type B , applied in vitro to the murine neuromuscular junction , interacts likewise with the motor nerve terminal except that a lower proportion of internalized radioactivity is seen .
	manualset3
96305	3	400790	13	NULL	NULL	0	NULL	motor nerve terminal 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	125I-BoNT type B , applied in vitro to the murine neuromuscular junction , interacts likewise with the motor nerve terminal except that a lower proportion of internalized radioactivity is seen .
	manualset3
96306	4	400790	13	NULL	NULL	0	NULL	lower proportion 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	125I-BoNT type B , applied in vitro to the murine neuromuscular junction , interacts likewise with the motor nerve terminal except that a lower proportion of internalized radioactivity is seen .
	manualset3
96307	5	400790	13	NULL	NULL	0	NULL	radioactivity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	125I-BoNT type B , applied in vitro to the murine neuromuscular junction , interacts likewise with the motor nerve terminal except that a lower proportion of internalized radioactivity is seen .
	manualset3
96308	1	400791	13	NULL	NULL	0	NULL	response times profiles	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In their response times profiles , the expected magnitude effect was systematically modified by properties of number signs in Korean sign language in a culture-specific way ( not observed in hearing and deaf Germans or hearing Chinese ) .
	manualset3
96309	2	400791	13	NULL	NULL	0	NULL	magnitude effect 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In their response times profiles , the expected magnitude effect was systematically modified by properties of number signs in Korean sign language in a culture-specific way ( not observed in hearing and deaf Germans or hearing Chinese ) .
	manualset3
96310	3	400791	13	NULL	NULL	0	NULL	properties of number signs	Language												NULL		0	NULL	NULL	NULL	NULL	NULL	In their response times profiles , the expected magnitude effect was systematically modified by properties of number signs in Korean sign language in a culture-specific way ( not observed in hearing and deaf Germans or hearing Chinese ) .
	manualset3
96311	4	400791	13	NULL	NULL	0	NULL	 Korean sign language 	Language												NULL		0	NULL	NULL	NULL	NULL	NULL	In their response times profiles , the expected magnitude effect was systematically modified by properties of number signs in Korean sign language in a culture-specific way ( not observed in hearing and deaf Germans or hearing Chinese ) .
	manualset3
96312	5	400791	13	NULL	NULL	0	NULL	culture-specific way	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In their response times profiles , the expected magnitude effect was systematically modified by properties of number signs in Korean sign language in a culture-specific way ( not observed in hearing and deaf Germans or hearing Chinese ) .
	manualset3
96313	6	400791	13	NULL	NULL	0	NULL	hearing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In their response times profiles , the expected magnitude effect was systematically modified by properties of number signs in Korean sign language in a culture-specific way ( not observed in hearing and deaf Germans or hearing Chinese ) .
	manualset3
96314	7	400791	13	NULL	NULL	0	NULL	deaf Germans	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In their response times profiles , the expected magnitude effect was systematically modified by properties of number signs in Korean sign language in a culture-specific way ( not observed in hearing and deaf Germans or hearing Chinese ) .
	manualset3
96315	8	400791	13	NULL	NULL	0	NULL	hearing Chinese 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In their response times profiles , the expected magnitude effect was systematically modified by properties of number signs in Korean sign language in a culture-specific way ( not observed in hearing and deaf Germans or hearing Chinese ) .
	manualset3
96316	1	400792	13	NULL	NULL	0	NULL	therapeutic experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In therapeutic experiments , a single low-dose ( 2 x 10 ( 7 ) plaque-forming units ) intratumoral injection of AdRGD-IL-12 elicited pronounced anti-tumor activity and notably prolonged the survival of Meth-A fibrosarcoma-bearing mice .
	manualset3
96317	2	400792	13	NULL	NULL	0	NULL	 2 x 10 ( 7 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In therapeutic experiments , a single low-dose ( 2 x 10 ( 7 ) plaque-forming units ) intratumoral injection of AdRGD-IL-12 elicited pronounced anti-tumor activity and notably prolonged the survival of Meth-A fibrosarcoma-bearing mice .
	manualset3
96318	3	400792	13	NULL	NULL	0	NULL	plaque-forming units	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In therapeutic experiments , a single low-dose ( 2 x 10 ( 7 ) plaque-forming units ) intratumoral injection of AdRGD-IL-12 elicited pronounced anti-tumor activity and notably prolonged the survival of Meth-A fibrosarcoma-bearing mice .
	manualset3
96319	4	400792	13	NULL	NULL	0	NULL	intratumoral injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In therapeutic experiments , a single low-dose ( 2 x 10 ( 7 ) plaque-forming units ) intratumoral injection of AdRGD-IL-12 elicited pronounced anti-tumor activity and notably prolonged the survival of Meth-A fibrosarcoma-bearing mice .
	manualset3
96320	5	400792	13	NULL	NULL	0	NULL	AdRGD-IL-12	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In therapeutic experiments , a single low-dose ( 2 x 10 ( 7 ) plaque-forming units ) intratumoral injection of AdRGD-IL-12 elicited pronounced anti-tumor activity and notably prolonged the survival of Meth-A fibrosarcoma-bearing mice .
	manualset3
96321	6	400792	13	NULL	NULL	0	NULL	 anti-tumor activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In therapeutic experiments , a single low-dose ( 2 x 10 ( 7 ) plaque-forming units ) intratumoral injection of AdRGD-IL-12 elicited pronounced anti-tumor activity and notably prolonged the survival of Meth-A fibrosarcoma-bearing mice .
	manualset3
96322	7	400792	13	NULL	NULL	0	NULL	survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In therapeutic experiments , a single low-dose ( 2 x 10 ( 7 ) plaque-forming units ) intratumoral injection of AdRGD-IL-12 elicited pronounced anti-tumor activity and notably prolonged the survival of Meth-A fibrosarcoma-bearing mice .
	manualset3
96323	8	400792	13	NULL	NULL	0	NULL	Meth-A fibrosarcoma-bearing mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In therapeutic experiments , a single low-dose ( 2 x 10 ( 7 ) plaque-forming units ) intratumoral injection of AdRGD-IL-12 elicited pronounced anti-tumor activity and notably prolonged the survival of Meth-A fibrosarcoma-bearing mice .
	manualset3
96324	1	400793	13	NULL	NULL	0	NULL	33 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In these 33 patients CPAP and APAP reduced the Epworth Sleepiness score from 15 + / -1 ( + / - SEM ) to 8 + / -1 and 9 + / -1 respectively ( both & lt ; 0.0001 from baseline but NS between modes ) .
	manualset3
96325	2	400793	13	NULL	NULL	0	NULL	CPAP	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In these 33 patients CPAP and APAP reduced the Epworth Sleepiness score from 15 + / -1 ( + / - SEM ) to 8 + / -1 and 9 + / -1 respectively ( both & lt ; 0.0001 from baseline but NS between modes ) .
	manualset3
96326	3	400793	13	NULL	NULL	0	NULL	APAP	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In these 33 patients CPAP and APAP reduced the Epworth Sleepiness score from 15 + / -1 ( + / - SEM ) to 8 + / -1 and 9 + / -1 respectively ( both & lt ; 0.0001 from baseline but NS between modes ) .
	manualset3
96327	4	400793	13	NULL	NULL	0	NULL	Epworth Sleepiness score	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In these 33 patients CPAP and APAP reduced the Epworth Sleepiness score from 15 + / -1 ( + / - SEM ) to 8 + / -1 and 9 + / -1 respectively ( both & lt ; 0.0001 from baseline but NS between modes ) .
	manualset3
96328	5	400793	13	NULL	NULL	0	NULL	15 + / -1 ( + / - SEM ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In these 33 patients CPAP and APAP reduced the Epworth Sleepiness score from 15 + / -1 ( + / - SEM ) to 8 + / -1 and 9 + / -1 respectively ( both & lt ; 0.0001 from baseline but NS between modes ) .
	manualset3
96329	6	400793	13	NULL	NULL	NULL	NULL	8 + / -1	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In these 33 patients CPAP and APAP reduced the Epworth Sleepiness score from 15 + / -1 ( + / - SEM ) to 8 + / -1 and 9 + / -1 respectively ( both & lt ; 0.0001 from baseline but NS between modes ) .
	manualset3
96330	7	400793	13	NULL	NULL	0	NULL	9 + / -1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In these 33 patients CPAP and APAP reduced the Epworth Sleepiness score from 15 + / -1 ( + / - SEM ) to 8 + / -1 and 9 + / -1 respectively ( both & lt ; 0.0001 from baseline but NS between modes ) .
	manualset3
96331	8	400793	13	NULL	NULL	NULL	NULL	both & lt ; 0.0001 from baseline but NS between modes 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In these 33 patients CPAP and APAP reduced the Epworth Sleepiness score from 15 + / -1 ( + / - SEM ) to 8 + / -1 and 9 + / -1 respectively ( both & lt ; 0.0001 from baseline but NS between modes ) .
	manualset3
96332	1	400794	13	NULL	NULL	0	NULL	birds	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In these birds , all neurons in the region of the FLC in which characteristic frequencies ( CFs ) normally increase from 2 to 6 kHz had CF in the range of 2-4 kHz .
	manualset3
96333	2	400794	13	NULL	NULL	0	NULL	neurons 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In these birds , all neurons in the region of the FLC in which characteristic frequencies ( CFs ) normally increase from 2 to 6 kHz had CF in the range of 2-4 kHz .
	manualset3
96334	3	400794	13	NULL	NULL	0	NULL	region of the FLC	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In these birds , all neurons in the region of the FLC in which characteristic frequencies ( CFs ) normally increase from 2 to 6 kHz had CF in the range of 2-4 kHz .
	manualset3
96335	4	400794	13	NULL	NULL	0	NULL	characteristic frequencies ( CFs )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In these birds , all neurons in the region of the FLC in which characteristic frequencies ( CFs ) normally increase from 2 to 6 kHz had CF in the range of 2-4 kHz .
	manualset3
96336	5	400794	13	NULL	NULL	0	NULL	2 to 6 kHz	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In these birds , all neurons in the region of the FLC in which characteristic frequencies ( CFs ) normally increase from 2 to 6 kHz had CF in the range of 2-4 kHz .
	manualset3
96337	6	400794	13	NULL	NULL	0	NULL	CF	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In these birds , all neurons in the region of the FLC in which characteristic frequencies ( CFs ) normally increase from 2 to 6 kHz had CF in the range of 2-4 kHz .
	manualset3
96338	7	400794	13	NULL	NULL	0	NULL	range of 2-4 kHz	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In these birds , all neurons in the region of the FLC in which characteristic frequencies ( CFs ) normally increase from 2 to 6 kHz had CF in the range of 2-4 kHz .
	manualset3
96510	1	400795	13	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In these cases with presence of characteristic lesions of GMB without positive family history the diagnosis Alport syndrome can not be established with certainty , further examinations are necessary .
	manualset3
96514	2	400795	13	NULL	NULL	0	NULL	presence of characteristic lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In these cases with presence of characteristic lesions of GMB without positive family history the diagnosis Alport syndrome can not be established with certainty , further examinations are necessary .
	manualset3
96519	3	400795	13	NULL	NULL	0	NULL	GMB	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In these cases with presence of characteristic lesions of GMB without positive family history the diagnosis Alport syndrome can not be established with certainty , further examinations are necessary .
	manualset3
96529	4	400795	13	NULL	NULL	0	NULL	positive family history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In these cases with presence of characteristic lesions of GMB without positive family history the diagnosis Alport syndrome can not be established with certainty , further examinations are necessary .
	manualset3
96532	5	400795	13	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In these cases with presence of characteristic lesions of GMB without positive family history the diagnosis Alport syndrome can not be established with certainty , further examinations are necessary .
	manualset3
96534	6	400795	13	NULL	NULL	0	NULL	Alport syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In these cases with presence of characteristic lesions of GMB without positive family history the diagnosis Alport syndrome can not be established with certainty , further examinations are necessary .
	manualset3
96538	7	400795	13	NULL	NULL	0	NULL	certainty	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In these cases with presence of characteristic lesions of GMB without positive family history the diagnosis Alport syndrome can not be established with certainty , further examinations are necessary .
	manualset3
96540	8	400795	13	NULL	NULL	0	NULL	examinations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In these cases with presence of characteristic lesions of GMB without positive family history the diagnosis Alport syndrome can not be established with certainty , further examinations are necessary .
	manualset3
96597	1	400796	13	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In these cells , the most modified organelles were intracytoplasmic membranes ( endoplasmic reticulum ) and microfilament arrangements .
	manualset3
96599	2	400796	13	NULL	NULL	0	NULL	organelles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In these cells , the most modified organelles were intracytoplasmic membranes ( endoplasmic reticulum ) and microfilament arrangements .
	manualset3
96601	3	400796	13	NULL	NULL	0	NULL	intracytoplasmic membranes 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In these cells , the most modified organelles were intracytoplasmic membranes ( endoplasmic reticulum ) and microfilament arrangements .
	manualset3
96603	4	400796	13	NULL	NULL	0	NULL	endoplasmic reticulum 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In these cells , the most modified organelles were intracytoplasmic membranes ( endoplasmic reticulum ) and microfilament arrangements .
	manualset3
96605	5	400796	13	NULL	NULL	0	NULL	microfilament arrangements	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In these cells , the most modified organelles were intracytoplasmic membranes ( endoplasmic reticulum ) and microfilament arrangements .
	manualset3
96606	1	400797	13	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In these cells , we found deletion of the exon 9-intron 9 boundary including the splicing donor site in E-cadherin genomic DNA .
	manualset3
96607	2	400797	13	NULL	NULL	0	NULL	exon 9-intron 9 boundary	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In these cells , we found deletion of the exon 9-intron 9 boundary including the splicing donor site in E-cadherin genomic DNA .
	manualset3
96608	3	400797	13	NULL	NULL	0	NULL	splicing donor site	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In these cells , we found deletion of the exon 9-intron 9 boundary including the splicing donor site in E-cadherin genomic DNA .
	manualset3
96609	4	400797	13	NULL	NULL	0	NULL	E-cadherin genomic DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In these cells , we found deletion of the exon 9-intron 9 boundary including the splicing donor site in E-cadherin genomic DNA .
	manualset3
98953	5	400797	13	NULL	NULL	0	NULL	deletion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In these cells , we found deletion of the exon 9-intron 9 boundary including the splicing donor site in E-cadherin genomic DNA .
	manualset3
96635	1	400798	13	NULL	NULL	0	NULL	experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In these experiments , neurovirulence was associated with a change from a serine to an arginine at position 195 and a glycine to an alanine at position 198 within the envelope protein .
	manualset3
96636	2	400798	13	NULL	NULL	0	NULL	neurovirulence 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In these experiments , neurovirulence was associated with a change from a serine to an arginine at position 195 and a glycine to an alanine at position 198 within the envelope protein .
	manualset3
96637	3	400798	13	NULL	NULL	0	NULL	change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In these experiments , neurovirulence was associated with a change from a serine to an arginine at position 195 and a glycine to an alanine at position 198 within the envelope protein .
	manualset3
96638	4	400798	13	NULL	NULL	0	NULL	 serine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In these experiments , neurovirulence was associated with a change from a serine to an arginine at position 195 and a glycine to an alanine at position 198 within the envelope protein .
	manualset3
96639	5	400798	13	NULL	NULL	0	NULL	arginine at position 195	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In these experiments , neurovirulence was associated with a change from a serine to an arginine at position 195 and a glycine to an alanine at position 198 within the envelope protein .
	manualset3
96640	6	400798	13	NULL	NULL	0	NULL	glycine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In these experiments , neurovirulence was associated with a change from a serine to an arginine at position 195 and a glycine to an alanine at position 198 within the envelope protein .
	manualset3
96641	7	400798	13	NULL	NULL	0	NULL	 alanine at position 198	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In these experiments , neurovirulence was associated with a change from a serine to an arginine at position 195 and a glycine to an alanine at position 198 within the envelope protein .
	manualset3
96642	8	400798	13	NULL	NULL	0	NULL	envelope protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In these experiments , neurovirulence was associated with a change from a serine to an arginine at position 195 and a glycine to an alanine at position 198 within the envelope protein .
	manualset3
96643	1	400799	13	NULL	NULL	0	NULL	thoracic procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In these extensive thoracic procedures , respiratory dysfunction may be significant , persisting in the postoperative period .
	manualset3
96644	2	400799	13	NULL	NULL	0	NULL	respiratory dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In these extensive thoracic procedures , respiratory dysfunction may be significant , persisting in the postoperative period .
	manualset3
96645	3	400799	13	NULL	NULL	0	NULL	postoperative period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In these extensive thoracic procedures , respiratory dysfunction may be significant , persisting in the postoperative period .
	manualset3
96646	1	400800	13	NULL	NULL	0	NULL	13 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	13 patients were found unsuitable for revascularisation .
	manualset3
96647	2	400800	13	NULL	NULL	0	NULL	 revascularisation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	13 patients were found unsuitable for revascularisation .
	manualset3
96648	1	400801	13	NULL	NULL	0	NULL	materials	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In these materials , the fillers react with acids during the setting process or they improve the mechanical properties by increasing physical resistance , thermal expansion coefficient and radiopacity in acrylic filling materials .
	manualset3
96649	2	400801	13	NULL	NULL	0	NULL	fillers 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In these materials , the fillers react with acids during the setting process or they improve the mechanical properties by increasing physical resistance , thermal expansion coefficient and radiopacity in acrylic filling materials .
	manualset3
96650	3	400801	13	NULL	NULL	0	NULL	acids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In these materials , the fillers react with acids during the setting process or they improve the mechanical properties by increasing physical resistance , thermal expansion coefficient and radiopacity in acrylic filling materials .
	manualset3
96651	4	400801	13	NULL	NULL	0	NULL	 setting process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In these materials , the fillers react with acids during the setting process or they improve the mechanical properties by increasing physical resistance , thermal expansion coefficient and radiopacity in acrylic filling materials .
	manualset3
96652	5	400801	13	NULL	NULL	0	NULL	 mechanical properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In these materials , the fillers react with acids during the setting process or they improve the mechanical properties by increasing physical resistance , thermal expansion coefficient and radiopacity in acrylic filling materials .
	manualset3
96653	6	400801	13	NULL	NULL	0	NULL	physical resistance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In these materials , the fillers react with acids during the setting process or they improve the mechanical properties by increasing physical resistance , thermal expansion coefficient and radiopacity in acrylic filling materials .
	manualset3
96654	7	400801	13	NULL	NULL	0	NULL	thermal expansion coefficient	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In these materials , the fillers react with acids during the setting process or they improve the mechanical properties by increasing physical resistance , thermal expansion coefficient and radiopacity in acrylic filling materials .
	manualset3
96655	8	400801	13	NULL	NULL	0	NULL	radiopacity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In these materials , the fillers react with acids during the setting process or they improve the mechanical properties by increasing physical resistance , thermal expansion coefficient and radiopacity in acrylic filling materials .
	manualset3
96656	9	400801	13	NULL	NULL	0	NULL	acrylic filling materials	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In these materials , the fillers react with acids during the setting process or they improve the mechanical properties by increasing physical resistance , thermal expansion coefficient and radiopacity in acrylic filling materials .
	manualset3
96657	1	400802	13	NULL	NULL	0	NULL	situations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In these situations , blood or even urine can be of poor interest .
	manualset3
96658	2	400802	13	NULL	NULL	NULL	NULL	blood	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In these situations , blood or even urine can be of poor interest .
	manualset3
96659	3	400802	13	NULL	NULL	0	NULL	urine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In these situations , blood or even urine can be of poor interest .
	manualset3
96660	4	400802	13	NULL	NULL	0	NULL	interest	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In these situations , blood or even urine can be of poor interest .
	manualset3
96661	1	400803	13	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In these studies 5-FU was administered during ( concomitant chemotherapy : C-CHEM ) or after ERT ( adjuvant chemotherapy : A-CHEM ) .
	manualset3
96662	2	400803	13	NULL	NULL	0	NULL	5-FU 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In these studies 5-FU was administered during ( concomitant chemotherapy : C-CHEM ) or after ERT ( adjuvant chemotherapy : A-CHEM ) .
	manualset3
96663	3	400803	13	NULL	NULL	0	NULL	concomitant chemotherapy : C-CHEM 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In these studies 5-FU was administered during ( concomitant chemotherapy : C-CHEM ) or after ERT ( adjuvant chemotherapy : A-CHEM ) .
	manualset3
96664	4	400803	13	NULL	NULL	0	NULL	 ERT ( adjuvant chemotherapy : A-CHEM	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In these studies 5-FU was administered during ( concomitant chemotherapy : C-CHEM ) or after ERT ( adjuvant chemotherapy : A-CHEM ) .
	manualset3
96665	1	400804	13	NULL	NULL	0	NULL	subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In these subjects , PTH was secreted in a dual fashion , with significant basal ( tonic ) secretion and PTH pulses approximately every 20 min .
	manualset3
96666	2	400804	13	NULL	NULL	0	NULL	PTH	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In these subjects , PTH was secreted in a dual fashion , with significant basal ( tonic ) secretion and PTH pulses approximately every 20 min .
	manualset3
96667	3	400804	13	NULL	NULL	0	NULL	 dual fashion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In these subjects , PTH was secreted in a dual fashion , with significant basal ( tonic ) secretion and PTH pulses approximately every 20 min .
	manualset3
96668	4	400804	13	NULL	NULL	0	NULL	basal ( tonic ) secretion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In these subjects , PTH was secreted in a dual fashion , with significant basal ( tonic ) secretion and PTH pulses approximately every 20 min .
	manualset3
96669	5	400804	13	NULL	NULL	0	NULL	PTH pulses 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In these subjects , PTH was secreted in a dual fashion , with significant basal ( tonic ) secretion and PTH pulses approximately every 20 min .
	manualset3
96670	6	400804	13	NULL	NULL	0	NULL	 20 min 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In these subjects , PTH was secreted in a dual fashion , with significant basal ( tonic ) secretion and PTH pulses approximately every 20 min .
	manualset3
96671	1	400805	13	NULL	NULL	0	NULL	two subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In these two subjects , antiarrhythmic concentrations of encainide ( greater than 265 ng/ml ) were at least fivefold higher than those sustained in the six extensive metabolizers during steady state oral therapy .
	manualset3
96672	2	400805	13	NULL	NULL	0	NULL	antiarrhythmic concentrations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In these two subjects , antiarrhythmic concentrations of encainide ( greater than 265 ng/ml ) were at least fivefold higher than those sustained in the six extensive metabolizers during steady state oral therapy .
	manualset3
96673	3	400805	13	NULL	NULL	0	NULL	 encainide 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In these two subjects , antiarrhythmic concentrations of encainide ( greater than 265 ng/ml ) were at least fivefold higher than those sustained in the six extensive metabolizers during steady state oral therapy .
	manualset3
96674	4	400805	13	NULL	NULL	0	NULL	265 ng/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In these two subjects , antiarrhythmic concentrations of encainide ( greater than 265 ng/ml ) were at least fivefold higher than those sustained in the six extensive metabolizers during steady state oral therapy .
	manualset3
96675	5	400805	13	NULL	NULL	0	NULL	 fivefold higher 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In these two subjects , antiarrhythmic concentrations of encainide ( greater than 265 ng/ml ) were at least fivefold higher than those sustained in the six extensive metabolizers during steady state oral therapy .
	manualset3
96676	6	400805	13	NULL	NULL	0	NULL	six extensive metabolizers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In these two subjects , antiarrhythmic concentrations of encainide ( greater than 265 ng/ml ) were at least fivefold higher than those sustained in the six extensive metabolizers during steady state oral therapy .
	manualset3
96677	7	400805	13	NULL	NULL	0	NULL	steady state oral therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In these two subjects , antiarrhythmic concentrations of encainide ( greater than 265 ng/ml ) were at least fivefold higher than those sustained in the six extensive metabolizers during steady state oral therapy .
	manualset3
96678	1	400806	13	NULL	NULL	0	NULL	Letter 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this Letter , we report the synthesis and properties of miRNA duplexes carrying biaryl units at the 5 ' - terminus of one strand .
	manualset3
96679	2	400806	13	NULL	NULL	0	NULL	synthesis of miRNA duplexes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this Letter , we report the synthesis and properties of miRNA duplexes carrying biaryl units at the 5 ' - terminus of one strand .
	manualset3
96680	3	400806	13	NULL	NULL	0	NULL	properties of miRNA duplexes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this Letter , we report the synthesis and properties of miRNA duplexes carrying biaryl units at the 5 ' - terminus of one strand .
	manualset3
96681	4	400806	13	NULL	NULL	0	NULL	biaryl units at the 5 ' - terminus of one strand	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this Letter , we report the synthesis and properties of miRNA duplexes carrying biaryl units at the 5 ' - terminus of one strand .
	manualset3
96682	1	400807	13	NULL	NULL	0	NULL	Medicaid cohort	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this Medicaid cohort , HF-related hospitalizations did not lead to improved HF therapy .
	manualset3
96683	2	400807	13	NULL	NULL	0	NULL	HF-related hospitalizations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this Medicaid cohort , HF-related hospitalizations did not lead to improved HF therapy .
	manualset3
96684	3	400807	13	NULL	NULL	0	NULL	HF therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this Medicaid cohort , HF-related hospitalizations did not lead to improved HF therapy .
	manualset3
96685	1	400808	13	NULL	NULL	0	NULL	 PCR method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this PCR method , the appearance of male - and bovine-specific bands was independent of the DNA concentration .
	manualset3
96686	2	400808	13	NULL	NULL	0	NULL	appearance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this PCR method , the appearance of male - and bovine-specific bands was independent of the DNA concentration .
	manualset3
96687	3	400808	13	NULL	NULL	0	NULL	 male - specific bands	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this PCR method , the appearance of male - and bovine-specific bands was independent of the DNA concentration .
	manualset3
96688	4	400808	13	NULL	NULL	0	NULL	bovine-specific bands	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this PCR method , the appearance of male - and bovine-specific bands was independent of the DNA concentration .
	manualset3
96689	5	400808	13	NULL	NULL	NULL	NULL	DNA concentration	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this PCR method , the appearance of male - and bovine-specific bands was independent of the DNA concentration .
	manualset3
96690	1	400809	13	NULL	NULL	0	NULL	Review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this Review , I discuss recent studies that reveal a more extensive role for E and ID proteins in the transcriptional networks that drive the differentiation of many lymphoid lineages , as well as new functions for these proteins in hematopoietic stem cells and their multipotent , but lymphoid-primed , progeny .
	manualset3
96691	2	400809	13	NULL	NULL	0	NULL	recent studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this Review , I discuss recent studies that reveal a more extensive role for E and ID proteins in the transcriptional networks that drive the differentiation of many lymphoid lineages , as well as new functions for these proteins in hematopoietic stem cells and their multipotent , but lymphoid-primed , progeny .
	manualset3
96692	3	400809	13	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this Review , I discuss recent studies that reveal a more extensive role for E and ID proteins in the transcriptional networks that drive the differentiation of many lymphoid lineages , as well as new functions for these proteins in hematopoietic stem cells and their multipotent , but lymphoid-primed , progeny .
	manualset3
96693	4	400809	13	NULL	NULL	0	NULL	E proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this Review , I discuss recent studies that reveal a more extensive role for E and ID proteins in the transcriptional networks that drive the differentiation of many lymphoid lineages , as well as new functions for these proteins in hematopoietic stem cells and their multipotent , but lymphoid-primed , progeny .
	manualset3
96694	5	400809	13	NULL	NULL	0	NULL	ID proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this Review , I discuss recent studies that reveal a more extensive role for E and ID proteins in the transcriptional networks that drive the differentiation of many lymphoid lineages , as well as new functions for these proteins in hematopoietic stem cells and their multipotent , but lymphoid-primed , progeny .
	manualset3
96695	6	400809	13	NULL	NULL	0	NULL	transcriptional networks	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this Review , I discuss recent studies that reveal a more extensive role for E and ID proteins in the transcriptional networks that drive the differentiation of many lymphoid lineages , as well as new functions for these proteins in hematopoietic stem cells and their multipotent , but lymphoid-primed , progeny .
	manualset3
96696	7	400809	13	NULL	NULL	0	NULL	drive	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this Review , I discuss recent studies that reveal a more extensive role for E and ID proteins in the transcriptional networks that drive the differentiation of many lymphoid lineages , as well as new functions for these proteins in hematopoietic stem cells and their multipotent , but lymphoid-primed , progeny .
	manualset3
96697	8	400809	13	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this Review , I discuss recent studies that reveal a more extensive role for E and ID proteins in the transcriptional networks that drive the differentiation of many lymphoid lineages , as well as new functions for these proteins in hematopoietic stem cells and their multipotent , but lymphoid-primed , progeny .
	manualset3
96698	9	400809	13	NULL	NULL	0	NULL	lymphoid lineages 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this Review , I discuss recent studies that reveal a more extensive role for E and ID proteins in the transcriptional networks that drive the differentiation of many lymphoid lineages , as well as new functions for these proteins in hematopoietic stem cells and their multipotent , but lymphoid-primed , progeny .
	manualset3
96699	10	400809	13	NULL	NULL	0	NULL	functions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this Review , I discuss recent studies that reveal a more extensive role for E and ID proteins in the transcriptional networks that drive the differentiation of many lymphoid lineages , as well as new functions for these proteins in hematopoietic stem cells and their multipotent , but lymphoid-primed , progeny .
	manualset3
96700	11	400809	13	NULL	NULL	0	NULL	 proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this Review , I discuss recent studies that reveal a more extensive role for E and ID proteins in the transcriptional networks that drive the differentiation of many lymphoid lineages , as well as new functions for these proteins in hematopoietic stem cells and their multipotent , but lymphoid-primed , progeny .
	manualset3
96701	12	400809	13	NULL	NULL	0	NULL	hematopoietic stem cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this Review , I discuss recent studies that reveal a more extensive role for E and ID proteins in the transcriptional networks that drive the differentiation of many lymphoid lineages , as well as new functions for these proteins in hematopoietic stem cells and their multipotent , but lymphoid-primed , progeny .
	manualset3
96702	13	400809	13	NULL	NULL	0	NULL	multipotent , but lymphoid-primed , progeny 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this Review , I discuss recent studies that reveal a more extensive role for E and ID proteins in the transcriptional networks that drive the differentiation of many lymphoid lineages , as well as new functions for these proteins in hematopoietic stem cells and their multipotent , but lymphoid-primed , progeny .
	manualset3
96703	1	400810	13	NULL	NULL	0	NULL	Review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this Review , we summarize the most relevant findings from these studies , highlighting the substantial variation in patient conditions , peritoneal dialysis practices and management of comorbidities encountered in different parts of the world .
	manualset3
96704	2	400810	13	NULL	NULL	0	NULL	findings 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this Review , we summarize the most relevant findings from these studies , highlighting the substantial variation in patient conditions , peritoneal dialysis practices and management of comorbidities encountered in different parts of the world .
	manualset3
96705	3	400810	13	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this Review , we summarize the most relevant findings from these studies , highlighting the substantial variation in patient conditions , peritoneal dialysis practices and management of comorbidities encountered in different parts of the world .
	manualset3
96706	4	400810	13	NULL	NULL	0	NULL	variation in patient conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this Review , we summarize the most relevant findings from these studies , highlighting the substantial variation in patient conditions , peritoneal dialysis practices and management of comorbidities encountered in different parts of the world .
	manualset3
96707	5	400810	13	NULL	NULL	0	NULL	peritoneal dialysis practices 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this Review , we summarize the most relevant findings from these studies , highlighting the substantial variation in patient conditions , peritoneal dialysis practices and management of comorbidities encountered in different parts of the world .
	manualset3
96708	6	400810	13	NULL	NULL	0	NULL	management of comorbidities 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this Review , we summarize the most relevant findings from these studies , highlighting the substantial variation in patient conditions , peritoneal dialysis practices and management of comorbidities encountered in different parts of the world .
	manualset3
96709	7	400810	13	NULL	NULL	0	NULL	different parts of the world	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this Review , we summarize the most relevant findings from these studies , highlighting the substantial variation in patient conditions , peritoneal dialysis practices and management of comorbidities encountered in different parts of the world .
	manualset3
96710	1	400811	13	NULL	NULL	0	NULL	analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this analysis , the canonical cyclin binding motif PSTAIRE of CDK2 is replaced by a novel DARTLRE motif and Thr160 residue , phosphorylation of which is required for positive regulation of CDK2 , is replaced by a tyrosine ( Tyr174 ) in ( Ta ) 5B2 .
	manualset3
96711	2	400811	13	NULL	NULL	0	NULL	canonical cyclin binding motif PSTAIRE	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this analysis , the canonical cyclin binding motif PSTAIRE of CDK2 is replaced by a novel DARTLRE motif and Thr160 residue , phosphorylation of which is required for positive regulation of CDK2 , is replaced by a tyrosine ( Tyr174 ) in ( Ta ) 5B2 .
	manualset3
96712	3	400811	13	NULL	NULL	0	NULL	CDK2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this analysis , the canonical cyclin binding motif PSTAIRE of CDK2 is replaced by a novel DARTLRE motif and Thr160 residue , phosphorylation of which is required for positive regulation of CDK2 , is replaced by a tyrosine ( Tyr174 ) in ( Ta ) 5B2 .
	manualset3
96713	4	400811	13	NULL	NULL	0	NULL	novel DARTLRE motif	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this analysis , the canonical cyclin binding motif PSTAIRE of CDK2 is replaced by a novel DARTLRE motif and Thr160 residue , phosphorylation of which is required for positive regulation of CDK2 , is replaced by a tyrosine ( Tyr174 ) in ( Ta ) 5B2 .
	manualset3
96714	5	400811	13	NULL	NULL	0	NULL	Thr160 residue	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this analysis , the canonical cyclin binding motif PSTAIRE of CDK2 is replaced by a novel DARTLRE motif and Thr160 residue , phosphorylation of which is required for positive regulation of CDK2 , is replaced by a tyrosine ( Tyr174 ) in ( Ta ) 5B2 .
	manualset3
96715	6	400811	13	NULL	NULL	0	NULL	phosphorylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this analysis , the canonical cyclin binding motif PSTAIRE of CDK2 is replaced by a novel DARTLRE motif and Thr160 residue , phosphorylation of which is required for positive regulation of CDK2 , is replaced by a tyrosine ( Tyr174 ) in ( Ta ) 5B2 .
	manualset3
96716	7	400811	13	NULL	NULL	0	NULL	 positive regulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this analysis , the canonical cyclin binding motif PSTAIRE of CDK2 is replaced by a novel DARTLRE motif and Thr160 residue , phosphorylation of which is required for positive regulation of CDK2 , is replaced by a tyrosine ( Tyr174 ) in ( Ta ) 5B2 .
	manualset3
96717	8	400811	13	NULL	NULL	0	NULL	CDK2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this analysis , the canonical cyclin binding motif PSTAIRE of CDK2 is replaced by a novel DARTLRE motif and Thr160 residue , phosphorylation of which is required for positive regulation of CDK2 , is replaced by a tyrosine ( Tyr174 ) in ( Ta ) 5B2 .
	manualset3
96718	9	400811	13	NULL	NULL	0	NULL	 tyrosine ( Tyr174 )	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this analysis , the canonical cyclin binding motif PSTAIRE of CDK2 is replaced by a novel DARTLRE motif and Thr160 residue , phosphorylation of which is required for positive regulation of CDK2 , is replaced by a tyrosine ( Tyr174 ) in ( Ta ) 5B2 .
	manualset3
96719	10	400811	13	NULL	NULL	0	NULL	( Ta ) 5B2 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this analysis , the canonical cyclin binding motif PSTAIRE of CDK2 is replaced by a novel DARTLRE motif and Thr160 residue , phosphorylation of which is required for positive regulation of CDK2 , is replaced by a tyrosine ( Tyr174 ) in ( Ta ) 5B2 .
	manualset3
96720	1	400812	13	NULL	NULL	0	NULL	animal model	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this animal model no clear signs of myocardial depression or evidence of right heart failure were observed .
	manualset3
96721	2	400812	13	NULL	NULL	0	NULL	signs of myocardial depression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this animal model no clear signs of myocardial depression or evidence of right heart failure were observed .
	manualset3
96722	3	400812	13	NULL	NULL	0	NULL	evidence of right heart failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this animal model no clear signs of myocardial depression or evidence of right heart failure were observed .
	manualset3
96723	1	400813	13	NULL	NULL	0	NULL	approach 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this approach , the recombinant clones from a P. vivax genomic library are screened with radiolabelled human and P. falciparum DNA .
	manualset3
96724	2	400813	13	NULL	NULL	0	NULL	recombinant clones	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this approach , the recombinant clones from a P. vivax genomic library are screened with radiolabelled human and P. falciparum DNA .
	manualset3
96725	3	400813	13	NULL	NULL	0	NULL	P. vivax genomic library	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this approach , the recombinant clones from a P. vivax genomic library are screened with radiolabelled human and P. falciparum DNA .
	manualset3
96726	4	400813	13	NULL	NULL	0	NULL	human DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this approach , the recombinant clones from a P. vivax genomic library are screened with radiolabelled human and P. falciparum DNA .
	manualset3
96727	5	400813	13	NULL	NULL	0	NULL	P. falciparum DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this approach , the recombinant clones from a P. vivax genomic library are screened with radiolabelled human and P. falciparum DNA .
	manualset3
96728	1	400814	13	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , Winner and Atkinson summarize current knowledge of the effects of air pollutants on plant growth and physiology , and indicate the new directions of research now under way in North America and Europe .
	manualset3
96729	2	400814	13	NULL	NULL	0	NULL	Winner	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , Winner and Atkinson summarize current knowledge of the effects of air pollutants on plant growth and physiology , and indicate the new directions of research now under way in North America and Europe .
	manualset3
96730	3	400814	13	NULL	NULL	0	NULL	Atkinson	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , Winner and Atkinson summarize current knowledge of the effects of air pollutants on plant growth and physiology , and indicate the new directions of research now under way in North America and Europe .
	manualset3
96731	4	400814	13	NULL	NULL	0	NULL	current knowledge 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , Winner and Atkinson summarize current knowledge of the effects of air pollutants on plant growth and physiology , and indicate the new directions of research now under way in North America and Europe .
	manualset3
96732	5	400814	13	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , Winner and Atkinson summarize current knowledge of the effects of air pollutants on plant growth and physiology , and indicate the new directions of research now under way in North America and Europe .
	manualset3
96733	6	400814	13	NULL	NULL	0	NULL	air pollutants 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , Winner and Atkinson summarize current knowledge of the effects of air pollutants on plant growth and physiology , and indicate the new directions of research now under way in North America and Europe .
	manualset3
96734	7	400814	13	NULL	NULL	0	NULL	 plant growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , Winner and Atkinson summarize current knowledge of the effects of air pollutants on plant growth and physiology , and indicate the new directions of research now under way in North America and Europe .
	manualset3
96735	8	400814	13	NULL	NULL	0	NULL	physiology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , Winner and Atkinson summarize current knowledge of the effects of air pollutants on plant growth and physiology , and indicate the new directions of research now under way in North America and Europe .
	manualset3
96736	9	400814	13	NULL	NULL	0	NULL	new directions of research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , Winner and Atkinson summarize current knowledge of the effects of air pollutants on plant growth and physiology , and indicate the new directions of research now under way in North America and Europe .
	manualset3
96737	10	400814	13	NULL	NULL	0	NULL	North America	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , Winner and Atkinson summarize current knowledge of the effects of air pollutants on plant growth and physiology , and indicate the new directions of research now under way in North America and Europe .
	manualset3
96738	11	400814	13	NULL	NULL	0	NULL	Europe	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , Winner and Atkinson summarize current knowledge of the effects of air pollutants on plant growth and physiology , and indicate the new directions of research now under way in North America and Europe .
	manualset3
96739	1	400815	13	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , in a chronological format , women 's and nursing history are juxtaposed with feminist movements .
	manualset3
96740	2	400815	13	NULL	NULL	0	NULL	chronological format 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , in a chronological format , women 's and nursing history are juxtaposed with feminist movements .
	manualset3
96741	3	400815	13	NULL	NULL	0	NULL	women 's history	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , in a chronological format , women 's and nursing history are juxtaposed with feminist movements .
	manualset3
96742	4	400815	13	NULL	NULL	0	NULL	nursing history	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , in a chronological format , women 's and nursing history are juxtaposed with feminist movements .
	manualset3
96743	5	400815	13	NULL	NULL	0	NULL	feminist movements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , in a chronological format , women 's and nursing history are juxtaposed with feminist movements .
	manualset3
96744	1	400816	13	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , quality control procedures which are followed in tuberculosis laboratory to ensure the quality assurance , have been reviewed .
	manualset3
96745	2	400816	13	NULL	NULL	0	NULL	quality control procedures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , quality control procedures which are followed in tuberculosis laboratory to ensure the quality assurance , have been reviewed .
	manualset3
96746	3	400816	13	NULL	NULL	0	NULL	 tuberculosis laboratory 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , quality control procedures which are followed in tuberculosis laboratory to ensure the quality assurance , have been reviewed .
	manualset3
96747	4	400816	13	NULL	NULL	0	NULL	quality assurance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , quality control procedures which are followed in tuberculosis laboratory to ensure the quality assurance , have been reviewed .
	manualset3
96748	1	400817	13	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the author summarizes the most recent studies published on cancer vaccines where immunological parameters were analyzed to assess immunogenicity and , most importantly , to establish correlations with clinical benefit .
	manualset3
96749	2	400817	13	NULL	NULL	0	NULL	 author	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the author summarizes the most recent studies published on cancer vaccines where immunological parameters were analyzed to assess immunogenicity and , most importantly , to establish correlations with clinical benefit .
	manualset3
96750	3	400817	13	NULL	NULL	NULL	NULL	recent studies	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this article , the author summarizes the most recent studies published on cancer vaccines where immunological parameters were analyzed to assess immunogenicity and , most importantly , to establish correlations with clinical benefit .
	manualset3
96751	4	400817	13	NULL	NULL	0	NULL	cancer vaccines	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the author summarizes the most recent studies published on cancer vaccines where immunological parameters were analyzed to assess immunogenicity and , most importantly , to establish correlations with clinical benefit .
	manualset3
96752	5	400817	13	NULL	NULL	0	NULL	immunological parameters 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the author summarizes the most recent studies published on cancer vaccines where immunological parameters were analyzed to assess immunogenicity and , most importantly , to establish correlations with clinical benefit .
	manualset3
96753	6	400817	13	NULL	NULL	0	NULL	immunogenicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the author summarizes the most recent studies published on cancer vaccines where immunological parameters were analyzed to assess immunogenicity and , most importantly , to establish correlations with clinical benefit .
	manualset3
96754	7	400817	13	NULL	NULL	0	NULL	 correlations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the author summarizes the most recent studies published on cancer vaccines where immunological parameters were analyzed to assess immunogenicity and , most importantly , to establish correlations with clinical benefit .
	manualset3
96755	8	400817	13	NULL	NULL	0	NULL	clinical benefit	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the author summarizes the most recent studies published on cancer vaccines where immunological parameters were analyzed to assess immunogenicity and , most importantly , to establish correlations with clinical benefit .
	manualset3
96756	1	400818	13	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the authors describe a case using a systematic approach to evaluating infrastructure for evidence-based practice and selecting an evidence-based practice model for application in an acute care organization , the University of Maryland Medical Center .
	manualset3
96757	2	400818	13	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the authors describe a case using a systematic approach to evaluating infrastructure for evidence-based practice and selecting an evidence-based practice model for application in an acute care organization , the University of Maryland Medical Center .
	manualset3
96758	3	400818	13	NULL	NULL	0	NULL	case	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the authors describe a case using a systematic approach to evaluating infrastructure for evidence-based practice and selecting an evidence-based practice model for application in an acute care organization , the University of Maryland Medical Center .
	manualset3
96759	4	400818	13	NULL	NULL	0	NULL	systematic approach 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the authors describe a case using a systematic approach to evaluating infrastructure for evidence-based practice and selecting an evidence-based practice model for application in an acute care organization , the University of Maryland Medical Center .
	manualset3
96760	5	400818	13	NULL	NULL	0	NULL	 infrastructure	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the authors describe a case using a systematic approach to evaluating infrastructure for evidence-based practice and selecting an evidence-based practice model for application in an acute care organization , the University of Maryland Medical Center .
	manualset3
96761	6	400818	13	NULL	NULL	0	NULL	evidence-based practice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the authors describe a case using a systematic approach to evaluating infrastructure for evidence-based practice and selecting an evidence-based practice model for application in an acute care organization , the University of Maryland Medical Center .
	manualset3
96762	7	400818	13	NULL	NULL	0	NULL	evidence-based practice model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the authors describe a case using a systematic approach to evaluating infrastructure for evidence-based practice and selecting an evidence-based practice model for application in an acute care organization , the University of Maryland Medical Center .
	manualset3
96763	8	400818	13	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the authors describe a case using a systematic approach to evaluating infrastructure for evidence-based practice and selecting an evidence-based practice model for application in an acute care organization , the University of Maryland Medical Center .
	manualset3
96764	9	400818	13	NULL	NULL	0	NULL	acute care organization	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the authors describe a case using a systematic approach to evaluating infrastructure for evidence-based practice and selecting an evidence-based practice model for application in an acute care organization , the University of Maryland Medical Center .
	manualset3
96765	10	400818	13	NULL	NULL	0	NULL	 University of Maryland Medical Center	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the authors describe a case using a systematic approach to evaluating infrastructure for evidence-based practice and selecting an evidence-based practice model for application in an acute care organization , the University of Maryland Medical Center .
	manualset3
96766	1	400819	13	NULL	NULL	0	NULL	1404 consecutive patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	1404 consecutive patients were included , 89 % completed the questionnaire ( n = 1250 ) .
	manualset3
96767	2	400819	13	NULL	NULL	0	NULL	89 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	1404 consecutive patients were included , 89 % completed the questionnaire ( n = 1250 ) .
	manualset3
96768	3	400819	13	NULL	NULL	NULL	NULL	questionnaire	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	1404 consecutive patients were included , 89 % completed the questionnaire ( n = 1250 ) .
	manualset3
96769	4	400819	13	NULL	NULL	0	NULL	 n = 1250	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	1404 consecutive patients were included , 89 % completed the questionnaire ( n = 1250 ) .
	manualset3
96771	1	400820	13	NULL	NULL	0	NULL	article 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the authors develop an exploratory synthesis of two qualitative studies in which they critique the lay-expert divide , suggesting instead a spectrum of knowledge ( s ) about health and scientific issues .
	manualset3
96772	2	400820	13	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the authors develop an exploratory synthesis of two qualitative studies in which they critique the lay-expert divide , suggesting instead a spectrum of knowledge ( s ) about health and scientific issues .
	manualset3
96773	3	400820	13	NULL	NULL	0	NULL	exploratory synthesis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the authors develop an exploratory synthesis of two qualitative studies in which they critique the lay-expert divide , suggesting instead a spectrum of knowledge ( s ) about health and scientific issues .
	manualset3
96774	4	400820	13	NULL	NULL	0	NULL	two qualitative studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the authors develop an exploratory synthesis of two qualitative studies in which they critique the lay-expert divide , suggesting instead a spectrum of knowledge ( s ) about health and scientific issues .
	manualset3
96775	5	400820	13	NULL	NULL	0	NULL	critique 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the authors develop an exploratory synthesis of two qualitative studies in which they critique the lay-expert divide , suggesting instead a spectrum of knowledge ( s ) about health and scientific issues .
	manualset3
96776	6	400820	13	NULL	NULL	0	NULL	spectrum of knowledge ( s )	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the authors develop an exploratory synthesis of two qualitative studies in which they critique the lay-expert divide , suggesting instead a spectrum of knowledge ( s ) about health and scientific issues .
	manualset3
96777	7	400820	13	NULL	NULL	0	NULL	health issues	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the authors develop an exploratory synthesis of two qualitative studies in which they critique the lay-expert divide , suggesting instead a spectrum of knowledge ( s ) about health and scientific issues .
	manualset3
96778	8	400820	13	NULL	NULL	0	NULL	scientific issues	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the authors develop an exploratory synthesis of two qualitative studies in which they critique the lay-expert divide , suggesting instead a spectrum of knowledge ( s ) about health and scientific issues .
	manualset3
96779	1	400821	13	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the authors summarize the findings on responsibilities for senior medical managers in hospitals , group practices , and managed care organizations .
	manualset3
96780	2	400821	13	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the authors summarize the findings on responsibilities for senior medical managers in hospitals , group practices , and managed care organizations .
	manualset3
96781	3	400821	13	NULL	NULL	0	NULL	findings	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the authors summarize the findings on responsibilities for senior medical managers in hospitals , group practices , and managed care organizations .
	manualset3
96782	4	400821	13	NULL	NULL	0	NULL	responsibilities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the authors summarize the findings on responsibilities for senior medical managers in hospitals , group practices , and managed care organizations .
	manualset3
96783	5	400821	13	NULL	NULL	0	NULL	senior medical managers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the authors summarize the findings on responsibilities for senior medical managers in hospitals , group practices , and managed care organizations .
	manualset3
96784	6	400821	13	NULL	NULL	0	NULL	hospitals	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the authors summarize the findings on responsibilities for senior medical managers in hospitals , group practices , and managed care organizations .
	manualset3
96785	7	400821	13	NULL	NULL	0	NULL	group practices	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the authors summarize the findings on responsibilities for senior medical managers in hospitals , group practices , and managed care organizations .
	manualset3
96786	8	400821	13	NULL	NULL	0	NULL	care organizations	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , the authors summarize the findings on responsibilities for senior medical managers in hospitals , group practices , and managed care organizations .
	manualset3
96787	1	400822	13	NULL	NULL	0	NULL	article 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we discuss the biological significance of alterations in the p53 tumor suppressor gene in cancers of the oesophagus and of the skin .
	manualset3
96788	2	400822	13	NULL	NULL	0	NULL	biological significance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we discuss the biological significance of alterations in the p53 tumor suppressor gene in cancers of the oesophagus and of the skin .
	manualset3
96789	3	400822	13	NULL	NULL	0	NULL	alterations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we discuss the biological significance of alterations in the p53 tumor suppressor gene in cancers of the oesophagus and of the skin .
	manualset3
96790	4	400822	13	NULL	NULL	0	NULL	p53 tumor suppressor gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we discuss the biological significance of alterations in the p53 tumor suppressor gene in cancers of the oesophagus and of the skin .
	manualset3
96791	5	400822	13	NULL	NULL	0	NULL	cancers of the oesophagus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we discuss the biological significance of alterations in the p53 tumor suppressor gene in cancers of the oesophagus and of the skin .
	manualset3
96792	6	400822	13	NULL	NULL	0	NULL	cancers of the skin 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we discuss the biological significance of alterations in the p53 tumor suppressor gene in cancers of the oesophagus and of the skin .
	manualset3
96793	1	400823	13	NULL	NULL	0	NULL	 article 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we focus on the innovative institutional mechanisms for popular involvement and accountability that are part of the architecture for governance of the SUS .
	manualset3
96794	2	400823	13	NULL	NULL	0	NULL	focus	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we focus on the innovative institutional mechanisms for popular involvement and accountability that are part of the architecture for governance of the SUS .
	manualset3
96795	3	400823	13	NULL	NULL	0	NULL	mechanisms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we focus on the innovative institutional mechanisms for popular involvement and accountability that are part of the architecture for governance of the SUS .
	manualset3
96796	4	400823	13	NULL	NULL	0	NULL	involvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we focus on the innovative institutional mechanisms for popular involvement and accountability that are part of the architecture for governance of the SUS .
	manualset3
96797	5	400823	13	NULL	NULL	0	NULL	accountability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we focus on the innovative institutional mechanisms for popular involvement and accountability that are part of the architecture for governance of the SUS .
	manualset3
96798	6	400823	13	NULL	NULL	0	NULL	part of the architecture	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we focus on the innovative institutional mechanisms for popular involvement and accountability that are part of the architecture for governance of the SUS .
	manualset3
96799	7	400823	13	NULL	NULL	0	NULL	governance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we focus on the innovative institutional mechanisms for popular involvement and accountability that are part of the architecture for governance of the SUS .
	manualset3
96800	8	400823	13	NULL	NULL	0	NULL	 SUS	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we focus on the innovative institutional mechanisms for popular involvement and accountability that are part of the architecture for governance of the SUS .
	manualset3
96801	1	400824	13	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we highlight state-of-the-art virus engineering principles and discuss recent advances that bring potential biomedical applications a step closer .
	manualset3
96802	2	400824	13	NULL	NULL	0	NULL	highlight 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we highlight state-of-the-art virus engineering principles and discuss recent advances that bring potential biomedical applications a step closer .
	manualset3
96803	3	400824	13	NULL	NULL	0	NULL	virus engineering principles	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we highlight state-of-the-art virus engineering principles and discuss recent advances that bring potential biomedical applications a step closer .
	manualset3
96804	4	400824	13	NULL	NULL	0	NULL	 recent advances 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we highlight state-of-the-art virus engineering principles and discuss recent advances that bring potential biomedical applications a step closer .
	manualset3
96805	5	400824	13	NULL	NULL	0	NULL	biomedical applications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we highlight state-of-the-art virus engineering principles and discuss recent advances that bring potential biomedical applications a step closer .
	manualset3
96806	1	400825	13	NULL	NULL	NULL	NULL	article	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this article , we review the protein families that are involved in interacting with and regulating cruciform structures , including ( a ) the junction-resolving enzymes , ( b ) DNA repair proteins and transcription factors , ( c ) proteins involved in replication and ( d ) chromatin-associated proteins .
	manualset3
96807	2	400825	13	NULL	NULL	0	NULL	review	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we review the protein families that are involved in interacting with and regulating cruciform structures , including ( a ) the junction-resolving enzymes , ( b ) DNA repair proteins and transcription factors , ( c ) proteins involved in replication and ( d ) chromatin-associated proteins .
	manualset3
96808	3	400825	13	NULL	NULL	0	NULL	protein families 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we review the protein families that are involved in interacting with and regulating cruciform structures , including ( a ) the junction-resolving enzymes , ( b ) DNA repair proteins and transcription factors , ( c ) proteins involved in replication and ( d ) chromatin-associated proteins .
	manualset3
96809	4	400825	13	NULL	NULL	0	NULL	interacting	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we review the protein families that are involved in interacting with and regulating cruciform structures , including ( a ) the junction-resolving enzymes , ( b ) DNA repair proteins and transcription factors , ( c ) proteins involved in replication and ( d ) chromatin-associated proteins .
	manualset3
96810	5	400825	13	NULL	NULL	0	NULL	cruciform structures	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we review the protein families that are involved in interacting with and regulating cruciform structures , including ( a ) the junction-resolving enzymes , ( b ) DNA repair proteins and transcription factors , ( c ) proteins involved in replication and ( d ) chromatin-associated proteins .
	manualset3
96811	6	400825	13	NULL	NULL	0	NULL	junction-resolving enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we review the protein families that are involved in interacting with and regulating cruciform structures , including ( a ) the junction-resolving enzymes , ( b ) DNA repair proteins and transcription factors , ( c ) proteins involved in replication and ( d ) chromatin-associated proteins .
	manualset3
96812	7	400825	13	NULL	NULL	0	NULL	DNA repair proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we review the protein families that are involved in interacting with and regulating cruciform structures , including ( a ) the junction-resolving enzymes , ( b ) DNA repair proteins and transcription factors , ( c ) proteins involved in replication and ( d ) chromatin-associated proteins .
	manualset3
96813	8	400825	13	NULL	NULL	0	NULL	transcription factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we review the protein families that are involved in interacting with and regulating cruciform structures , including ( a ) the junction-resolving enzymes , ( b ) DNA repair proteins and transcription factors , ( c ) proteins involved in replication and ( d ) chromatin-associated proteins .
	manualset3
96814	9	400825	13	NULL	NULL	0	NULL	 proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we review the protein families that are involved in interacting with and regulating cruciform structures , including ( a ) the junction-resolving enzymes , ( b ) DNA repair proteins and transcription factors , ( c ) proteins involved in replication and ( d ) chromatin-associated proteins .
	manualset3
96815	10	400825	13	NULL	NULL	0	NULL	replication 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we review the protein families that are involved in interacting with and regulating cruciform structures , including ( a ) the junction-resolving enzymes , ( b ) DNA repair proteins and transcription factors , ( c ) proteins involved in replication and ( d ) chromatin-associated proteins .
	manualset3
96816	11	400825	13	NULL	NULL	0	NULL	chromatin-associated proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we review the protein families that are involved in interacting with and regulating cruciform structures , including ( a ) the junction-resolving enzymes , ( b ) DNA repair proteins and transcription factors , ( c ) proteins involved in replication and ( d ) chromatin-associated proteins .
	manualset3
96817	1	400826	13	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article I contrast two alternative frameworks , the deterministic and the probabilistic as competing paths to achieve successful quantitative immune models .
	manualset3
96818	2	400826	13	NULL	NULL	0	NULL	two alternative frameworks	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article I contrast two alternative frameworks , the deterministic and the probabilistic as competing paths to achieve successful quantitative immune models .
	manualset3
96819	3	400826	13	NULL	NULL	0	NULL	paths	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article I contrast two alternative frameworks , the deterministic and the probabilistic as competing paths to achieve successful quantitative immune models .
	manualset3
96820	4	400826	13	NULL	NULL	NULL	NULL	quantitative immune models	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this article I contrast two alternative frameworks , the deterministic and the probabilistic as competing paths to achieve successful quantitative immune models .
	manualset3
96821	1	400827	13	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article and its companion , we present our study of the characteristics of competence and expertise in the field of oral surgery .
	manualset3
96822	2	400827	13	NULL	NULL	0	NULL	companion	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article and its companion , we present our study of the characteristics of competence and expertise in the field of oral surgery .
	manualset3
96823	3	400827	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article and its companion , we present our study of the characteristics of competence and expertise in the field of oral surgery .
	manualset3
96824	4	400827	13	NULL	NULL	0	NULL	characteristics of competence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article and its companion , we present our study of the characteristics of competence and expertise in the field of oral surgery .
	manualset3
96825	5	400827	13	NULL	NULL	0	NULL	characteristics of expertise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article and its companion , we present our study of the characteristics of competence and expertise in the field of oral surgery .
	manualset3
96826	6	400827	13	NULL	NULL	0	NULL	field of oral surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article and its companion , we present our study of the characteristics of competence and expertise in the field of oral surgery .
	manualset3
96827	1	400828	13	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article we review the major mechanisms controlling angiogenesis and its role during endochondral ossification .
	manualset3
96828	2	400828	13	NULL	NULL	0	NULL	review 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article we review the major mechanisms controlling angiogenesis and its role during endochondral ossification .
	manualset3
96829	3	400828	13	NULL	NULL	0	NULL	major mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article we review the major mechanisms controlling angiogenesis and its role during endochondral ossification .
	manualset3
96830	4	400828	13	NULL	NULL	0	NULL	 angiogenesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article we review the major mechanisms controlling angiogenesis and its role during endochondral ossification .
	manualset3
96831	5	400828	13	NULL	NULL	0	NULL	role 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article we review the major mechanisms controlling angiogenesis and its role during endochondral ossification .
	manualset3
96832	6	400828	13	NULL	NULL	0	NULL	endochondral ossification	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article we review the major mechanisms controlling angiogenesis and its role during endochondral ossification .
	manualset3
96833	1	400829	13	NULL	NULL	0	NULL	article 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article we summarise the basic biology of fracture healing .
	manualset3
96834	2	400829	13	NULL	NULL	0	NULL	basic biology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article we summarise the basic biology of fracture healing .
	manualset3
96835	3	400829	13	NULL	NULL	0	NULL	fracture healing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article we summarise the basic biology of fracture healing .
	manualset3
96836	1	400830	13	NULL	NULL	0	NULL	assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this assay a peptide derived from p34cdc2 , cdc2 ( 6-20 ) NH2 , is coupled to the wells of a maleic anhydride-activated microtiter plate .
	manualset3
96837	2	400830	13	NULL	NULL	0	NULL	peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	In this assay a peptide derived from p34cdc2 , cdc2 ( 6-20 ) NH2 , is coupled to the wells of a maleic anhydride-activated microtiter plate .
	manualset3
96838	3	400830	13	NULL	NULL	0	NULL	p34cdc2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this assay a peptide derived from p34cdc2 , cdc2 ( 6-20 ) NH2 , is coupled to the wells of a maleic anhydride-activated microtiter plate .
	manualset3
96839	4	400830	13	NULL	NULL	0	NULL	cdc2 ( 6-20 ) NH2	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this assay a peptide derived from p34cdc2 , cdc2 ( 6-20 ) NH2 , is coupled to the wells of a maleic anhydride-activated microtiter plate .
	manualset3
96840	5	400830	13	NULL	NULL	0	NULL	wells	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this assay a peptide derived from p34cdc2 , cdc2 ( 6-20 ) NH2 , is coupled to the wells of a maleic anhydride-activated microtiter plate .
	manualset3
96841	6	400830	13	NULL	NULL	0	NULL	maleic anhydride-activated microtiter plate	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this assay a peptide derived from p34cdc2 , cdc2 ( 6-20 ) NH2 , is coupled to the wells of a maleic anhydride-activated microtiter plate .
	manualset3
96844	1	400831	13	NULL	NULL	0	NULL	brief overview	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this brief overview various neurochemical isolation procedures that can be adopted for the analysis of several monoamine neurotransmitters/neuromodulators and their principal oxidatively deaminated metabolites are outlined .
	manualset3
96845	2	400831	13	NULL	NULL	0	NULL	neurochemical isolation procedures	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this brief overview various neurochemical isolation procedures that can be adopted for the analysis of several monoamine neurotransmitters/neuromodulators and their principal oxidatively deaminated metabolites are outlined .
	manualset3
96846	3	400831	13	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this brief overview various neurochemical isolation procedures that can be adopted for the analysis of several monoamine neurotransmitters/neuromodulators and their principal oxidatively deaminated metabolites are outlined .
	manualset3
96847	4	400831	13	NULL	NULL	0	NULL	monoamine neurotransmitters	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this brief overview various neurochemical isolation procedures that can be adopted for the analysis of several monoamine neurotransmitters/neuromodulators and their principal oxidatively deaminated metabolites are outlined .
	manualset3
96848	5	400831	13	NULL	NULL	NULL	NULL	monoamine neuromodulators  	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this brief overview various neurochemical isolation procedures that can be adopted for the analysis of several monoamine neurotransmitters/neuromodulators and their principal oxidatively deaminated metabolites are outlined .
	manualset3
96849	6	400831	13	NULL	NULL	0	NULL	metabolites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this brief overview various neurochemical isolation procedures that can be adopted for the analysis of several monoamine neurotransmitters/neuromodulators and their principal oxidatively deaminated metabolites are outlined .
	manualset3
96850	1	400832	13	NULL	NULL	0	NULL	case-control study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case-control study , polymorphism at IL-1RN VNTR was investigated using the allele-specific polymerase chain reaction method , while the polymerase chain reaction-restriction fragment length polymorphism technique was used to identify the TNFB +252 A/G genotype in 675 Brazilian individuals ( 229 with chronic gastritis ( CG ) , 200 with gastric cancer ( GC ) and 246 healthy individuals as controls ( C ) ) .
	manualset3
96851	2	400832	13	NULL	NULL	0	NULL	polymorphism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case-control study , polymorphism at IL-1RN VNTR was investigated using the allele-specific polymerase chain reaction method , while the polymerase chain reaction-restriction fragment length polymorphism technique was used to identify the TNFB +252 A/G genotype in 675 Brazilian individuals ( 229 with chronic gastritis ( CG ) , 200 with gastric cancer ( GC ) and 246 healthy individuals as controls ( C ) ) .
	manualset3
96852	3	400832	13	NULL	NULL	0	NULL	IL-1RN VNTR 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case-control study , polymorphism at IL-1RN VNTR was investigated using the allele-specific polymerase chain reaction method , while the polymerase chain reaction-restriction fragment length polymorphism technique was used to identify the TNFB +252 A/G genotype in 675 Brazilian individuals ( 229 with chronic gastritis ( CG ) , 200 with gastric cancer ( GC ) and 246 healthy individuals as controls ( C ) ) .
	manualset3
96853	4	400832	13	NULL	NULL	0	NULL	allele-specific polymerase chain reaction method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case-control study , polymorphism at IL-1RN VNTR was investigated using the allele-specific polymerase chain reaction method , while the polymerase chain reaction-restriction fragment length polymorphism technique was used to identify the TNFB +252 A/G genotype in 675 Brazilian individuals ( 229 with chronic gastritis ( CG ) , 200 with gastric cancer ( GC ) and 246 healthy individuals as controls ( C ) ) .
	manualset3
96854	5	400832	13	NULL	NULL	0	NULL	polymerase chain reaction-restriction fragment length polymorphism technique 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case-control study , polymorphism at IL-1RN VNTR was investigated using the allele-specific polymerase chain reaction method , while the polymerase chain reaction-restriction fragment length polymorphism technique was used to identify the TNFB +252 A/G genotype in 675 Brazilian individuals ( 229 with chronic gastritis ( CG ) , 200 with gastric cancer ( GC ) and 246 healthy individuals as controls ( C ) ) .
	manualset3
96855	6	400832	13	NULL	NULL	0	NULL	TNFB +252 A/G genotype	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case-control study , polymorphism at IL-1RN VNTR was investigated using the allele-specific polymerase chain reaction method , while the polymerase chain reaction-restriction fragment length polymorphism technique was used to identify the TNFB +252 A/G genotype in 675 Brazilian individuals ( 229 with chronic gastritis ( CG ) , 200 with gastric cancer ( GC ) and 246 healthy individuals as controls ( C ) ) .
	manualset3
96856	7	400832	13	NULL	NULL	0	NULL	675 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case-control study , polymorphism at IL-1RN VNTR was investigated using the allele-specific polymerase chain reaction method , while the polymerase chain reaction-restriction fragment length polymorphism technique was used to identify the TNFB +252 A/G genotype in 675 Brazilian individuals ( 229 with chronic gastritis ( CG ) , 200 with gastric cancer ( GC ) and 246 healthy individuals as controls ( C ) ) .
	manualset3
96857	8	400832	13	NULL	NULL	0	NULL	Brazilian individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case-control study , polymorphism at IL-1RN VNTR was investigated using the allele-specific polymerase chain reaction method , while the polymerase chain reaction-restriction fragment length polymorphism technique was used to identify the TNFB +252 A/G genotype in 675 Brazilian individuals ( 229 with chronic gastritis ( CG ) , 200 with gastric cancer ( GC ) and 246 healthy individuals as controls ( C ) ) .
	manualset3
96858	9	400832	13	NULL	NULL	0	NULL	229 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case-control study , polymorphism at IL-1RN VNTR was investigated using the allele-specific polymerase chain reaction method , while the polymerase chain reaction-restriction fragment length polymorphism technique was used to identify the TNFB +252 A/G genotype in 675 Brazilian individuals ( 229 with chronic gastritis ( CG ) , 200 with gastric cancer ( GC ) and 246 healthy individuals as controls ( C ) ) .
	manualset3
96859	10	400832	13	NULL	NULL	0	NULL	chronic gastritis ( CG )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case-control study , polymorphism at IL-1RN VNTR was investigated using the allele-specific polymerase chain reaction method , while the polymerase chain reaction-restriction fragment length polymorphism technique was used to identify the TNFB +252 A/G genotype in 675 Brazilian individuals ( 229 with chronic gastritis ( CG ) , 200 with gastric cancer ( GC ) and 246 healthy individuals as controls ( C ) ) .
	manualset3
96860	11	400832	13	NULL	NULL	NULL	NULL	200	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this case-control study , polymorphism at IL-1RN VNTR was investigated using the allele-specific polymerase chain reaction method , while the polymerase chain reaction-restriction fragment length polymorphism technique was used to identify the TNFB +252 A/G genotype in 675 Brazilian individuals ( 229 with chronic gastritis ( CG ) , 200 with gastric cancer ( GC ) and 246 healthy individuals as controls ( C ) ) .
	manualset3
96861	12	400832	13	NULL	NULL	0	NULL	gastric cancer ( GC )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case-control study , polymorphism at IL-1RN VNTR was investigated using the allele-specific polymerase chain reaction method , while the polymerase chain reaction-restriction fragment length polymorphism technique was used to identify the TNFB +252 A/G genotype in 675 Brazilian individuals ( 229 with chronic gastritis ( CG ) , 200 with gastric cancer ( GC ) and 246 healthy individuals as controls ( C ) ) .
	manualset3
96862	13	400832	13	NULL	NULL	0	NULL	246	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case-control study , polymorphism at IL-1RN VNTR was investigated using the allele-specific polymerase chain reaction method , while the polymerase chain reaction-restriction fragment length polymorphism technique was used to identify the TNFB +252 A/G genotype in 675 Brazilian individuals ( 229 with chronic gastritis ( CG ) , 200 with gastric cancer ( GC ) and 246 healthy individuals as controls ( C ) ) .
	manualset3
96863	14	400832	13	NULL	NULL	0	NULL	healthy individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case-control study , polymorphism at IL-1RN VNTR was investigated using the allele-specific polymerase chain reaction method , while the polymerase chain reaction-restriction fragment length polymorphism technique was used to identify the TNFB +252 A/G genotype in 675 Brazilian individuals ( 229 with chronic gastritis ( CG ) , 200 with gastric cancer ( GC ) and 246 healthy individuals as controls ( C ) ) .
	manualset3
96864	15	400832	13	NULL	NULL	0	NULL	controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case-control study , polymorphism at IL-1RN VNTR was investigated using the allele-specific polymerase chain reaction method , while the polymerase chain reaction-restriction fragment length polymorphism technique was used to identify the TNFB +252 A/G genotype in 675 Brazilian individuals ( 229 with chronic gastritis ( CG ) , 200 with gastric cancer ( GC ) and 246 healthy individuals as controls ( C ) ) .
	manualset3
96865	1	400833	13	NULL	NULL	0	NULL	case	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case , the ATP level increased , but to a level still lower than existed before exposure to glucose .
	manualset3
96866	2	400833	13	NULL	NULL	0	NULL	ATP level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case , the ATP level increased , but to a level still lower than existed before exposure to glucose .
	manualset3
96867	3	400833	13	NULL	NULL	0	NULL	 level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case , the ATP level increased , but to a level still lower than existed before exposure to glucose .
	manualset3
96868	4	400833	13	NULL	NULL	0	NULL	exposure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case , the ATP level increased , but to a level still lower than existed before exposure to glucose .
	manualset3
96869	5	400833	13	NULL	NULL	0	NULL	glucose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case , the ATP level increased , but to a level still lower than existed before exposure to glucose .
	manualset3
96870	1	400834	13	NULL	NULL	0	NULL	case	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case , the crystals were additionally protected by B. sphaericus exosporium .
	manualset3
96871	2	400834	13	NULL	NULL	0	NULL	crystals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case , the crystals were additionally protected by B. sphaericus exosporium .
	manualset3
96872	3	400834	13	NULL	NULL	0	NULL	B. sphaericus exosporium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case , the crystals were additionally protected by B. sphaericus exosporium .
	manualset3
96873	1	400835	13	NULL	NULL	0	NULL	case	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case , the presence of KCl at low and moderate concentrations provoked swelling , which rapidly turned on particle disintegration due to the weakness of chitosan-TPP ionic interactions .
	manualset3
96874	2	400835	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case , the presence of KCl at low and moderate concentrations provoked swelling , which rapidly turned on particle disintegration due to the weakness of chitosan-TPP ionic interactions .
	manualset3
96875	3	400835	13	NULL	NULL	0	NULL	 KCl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case , the presence of KCl at low and moderate concentrations provoked swelling , which rapidly turned on particle disintegration due to the weakness of chitosan-TPP ionic interactions .
	manualset3
96876	4	400835	13	NULL	NULL	0	NULL	concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case , the presence of KCl at low and moderate concentrations provoked swelling , which rapidly turned on particle disintegration due to the weakness of chitosan-TPP ionic interactions .
	manualset3
96877	5	400835	13	NULL	NULL	0	NULL	particle disintegration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case , the presence of KCl at low and moderate concentrations provoked swelling , which rapidly turned on particle disintegration due to the weakness of chitosan-TPP ionic interactions .
	manualset3
96879	7	400835	13	NULL	NULL	0	NULL	 chitosan-TPP ionic interactions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case , the presence of KCl at low and moderate concentrations provoked swelling , which rapidly turned on particle disintegration due to the weakness of chitosan-TPP ionic interactions .
	manualset3
98954	8	400835	13	NULL	NULL	0	NULL	swelling	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case , the presence of KCl at low and moderate concentrations provoked swelling , which rapidly turned on particle disintegration due to the weakness of chitosan-TPP ionic interactions .
	manualset3
96878	1	400836	13	NULL	NULL	NULL	NULL	case report 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this case report , an implant is placed into a healed mandibular ridge several months after extraction of the tooth .
	manualset3
96880	2	400836	13	NULL	NULL	0	NULL	implant	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case report , an implant is placed into a healed mandibular ridge several months after extraction of the tooth .
	manualset3
96881	3	400836	13	NULL	NULL	0	NULL	mandibular ridge	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case report , an implant is placed into a healed mandibular ridge several months after extraction of the tooth .
	manualset3
96882	4	400836	13	NULL	NULL	0	NULL	several months	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case report , an implant is placed into a healed mandibular ridge several months after extraction of the tooth .
	manualset3
96883	5	400836	13	NULL	NULL	0	NULL	extraction	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case report , an implant is placed into a healed mandibular ridge several months after extraction of the tooth .
	manualset3
96884	6	400836	13	NULL	NULL	0	NULL	tooth	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this case report , an implant is placed into a healed mandibular ridge several months after extraction of the tooth .
	manualset3
96885	1	400837	13	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Apropos of the development and surgical treatment of gastric schwannomas ) .
	manualset3
96886	2	400837	13	NULL	NULL	0	NULL	surgical treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Apropos of the development and surgical treatment of gastric schwannomas ) .
	manualset3
96887	3	400837	13	NULL	NULL	0	NULL	gastric schwannomas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Apropos of the development and surgical treatment of gastric schwannomas ) .
	manualset3
96888	1	400838	13	NULL	NULL	0	NULL	 chapter	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter , we describe a method to significantly enrich for myoblasts using - melanoma cell adhesion molecule ( MCAM ) , which we have determined to be an excellent marker of human fetal myoblasts .
	manualset3
96889	2	400838	13	NULL	NULL	0	NULL	method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter , we describe a method to significantly enrich for myoblasts using - melanoma cell adhesion molecule ( MCAM ) , which we have determined to be an excellent marker of human fetal myoblasts .
	manualset3
96890	3	400838	13	NULL	NULL	0	NULL	myoblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter , we describe a method to significantly enrich for myoblasts using - melanoma cell adhesion molecule ( MCAM ) , which we have determined to be an excellent marker of human fetal myoblasts .
	manualset3
96891	4	400838	13	NULL	NULL	0	NULL	melanoma cell adhesion molecule ( MCAM )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter , we describe a method to significantly enrich for myoblasts using - melanoma cell adhesion molecule ( MCAM ) , which we have determined to be an excellent marker of human fetal myoblasts .
	manualset3
96892	5	400838	13	NULL	NULL	0	NULL	excellent marker	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter , we describe a method to significantly enrich for myoblasts using - melanoma cell adhesion molecule ( MCAM ) , which we have determined to be an excellent marker of human fetal myoblasts .
	manualset3
96893	6	400838	13	NULL	NULL	0	NULL	 human fetal myoblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter , we describe a method to significantly enrich for myoblasts using - melanoma cell adhesion molecule ( MCAM ) , which we have determined to be an excellent marker of human fetal myoblasts .
	manualset3
96894	1	400839	13	NULL	NULL	0	NULL	chapter 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter , we describe a novel R. capsulatus expression system and its application .
	manualset3
96895	2	400839	13	NULL	NULL	0	NULL	novel R. capsulatus expression system	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter , we describe a novel R. capsulatus expression system and its application .
	manualset3
96896	3	400839	13	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter , we describe a novel R. capsulatus expression system and its application .
	manualset3
96897	1	400840	13	NULL	NULL	0	NULL	chapter	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter , we describe the structure of the wild-type p53 protein and present structural and functional data that provide the molecular basis for understanding the effects of common cancer mutations .
	manualset3
96898	2	400840	13	NULL	NULL	0	NULL	structure	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter , we describe the structure of the wild-type p53 protein and present structural and functional data that provide the molecular basis for understanding the effects of common cancer mutations .
	manualset3
96899	3	400840	13	NULL	NULL	0	NULL	wild-type p53 protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter , we describe the structure of the wild-type p53 protein and present structural and functional data that provide the molecular basis for understanding the effects of common cancer mutations .
	manualset3
96900	4	400840	13	NULL	NULL	0	NULL	structural data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter , we describe the structure of the wild-type p53 protein and present structural and functional data that provide the molecular basis for understanding the effects of common cancer mutations .
	manualset3
96901	5	400840	13	NULL	NULL	0	NULL	functional data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter , we describe the structure of the wild-type p53 protein and present structural and functional data that provide the molecular basis for understanding the effects of common cancer mutations .
	manualset3
96902	6	400840	13	NULL	NULL	NULL	NULL	molecular basis 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this chapter , we describe the structure of the wild-type p53 protein and present structural and functional data that provide the molecular basis for understanding the effects of common cancer mutations .
	manualset3
96903	7	400840	13	NULL	NULL	0	NULL	 effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter , we describe the structure of the wild-type p53 protein and present structural and functional data that provide the molecular basis for understanding the effects of common cancer mutations .
	manualset3
96904	8	400840	13	NULL	NULL	0	NULL	cancer mutations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter , we describe the structure of the wild-type p53 protein and present structural and functional data that provide the molecular basis for understanding the effects of common cancer mutations .
	manualset3
96905	1	400841	13	NULL	NULL	0	NULL	chapter 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter , we will summarize the mouse models that have allowed us to faithfully recapitulate features of human cancers and to highlight the network of connections between the PTEN signaling cascade and other oncogenic or tumor suppressive pathways .
	manualset3
96906	2	400841	13	NULL	NULL	0	NULL	mouse models	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter , we will summarize the mouse models that have allowed us to faithfully recapitulate features of human cancers and to highlight the network of connections between the PTEN signaling cascade and other oncogenic or tumor suppressive pathways .
	manualset3
96907	3	400841	13	NULL	NULL	0	NULL	features of human cancers	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter , we will summarize the mouse models that have allowed us to faithfully recapitulate features of human cancers and to highlight the network of connections between the PTEN signaling cascade and other oncogenic or tumor suppressive pathways .
	manualset3
96908	4	400841	13	NULL	NULL	0	NULL	highlight	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter , we will summarize the mouse models that have allowed us to faithfully recapitulate features of human cancers and to highlight the network of connections between the PTEN signaling cascade and other oncogenic or tumor suppressive pathways .
	manualset3
96909	5	400841	13	NULL	NULL	0	NULL	network of connections	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter , we will summarize the mouse models that have allowed us to faithfully recapitulate features of human cancers and to highlight the network of connections between the PTEN signaling cascade and other oncogenic or tumor suppressive pathways .
	manualset3
96910	6	400841	13	NULL	NULL	0	NULL	PTEN signaling cascade	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter , we will summarize the mouse models that have allowed us to faithfully recapitulate features of human cancers and to highlight the network of connections between the PTEN signaling cascade and other oncogenic or tumor suppressive pathways .
	manualset3
96911	7	400841	13	NULL	NULL	0	NULL	oncogenic pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter , we will summarize the mouse models that have allowed us to faithfully recapitulate features of human cancers and to highlight the network of connections between the PTEN signaling cascade and other oncogenic or tumor suppressive pathways .
	manualset3
96912	8	400841	13	NULL	NULL	0	NULL	tumor suppressive pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter , we will summarize the mouse models that have allowed us to faithfully recapitulate features of human cancers and to highlight the network of connections between the PTEN signaling cascade and other oncogenic or tumor suppressive pathways .
	manualset3
96913	1	400842	13	NULL	NULL	0	NULL	chapter 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter we discuss study protocols aimed at integrating in vitro preparation of cells , small animal surgery , behavioral testing batteries , and histological analysis .
	manualset3
96914	2	400842	13	NULL	NULL	0	NULL	study protocols	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter we discuss study protocols aimed at integrating in vitro preparation of cells , small animal surgery , behavioral testing batteries , and histological analysis .
	manualset3
96915	3	400842	13	NULL	NULL	0	NULL	in vitro preparation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter we discuss study protocols aimed at integrating in vitro preparation of cells , small animal surgery , behavioral testing batteries , and histological analysis .
	manualset3
96916	4	400842	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter we discuss study protocols aimed at integrating in vitro preparation of cells , small animal surgery , behavioral testing batteries , and histological analysis .
	manualset3
96917	5	400842	13	NULL	NULL	0	NULL	 small animal surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter we discuss study protocols aimed at integrating in vitro preparation of cells , small animal surgery , behavioral testing batteries , and histological analysis .
	manualset3
96918	6	400842	13	NULL	NULL	0	NULL	behavioral testing batteries	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter we discuss study protocols aimed at integrating in vitro preparation of cells , small animal surgery , behavioral testing batteries , and histological analysis .
	manualset3
96919	7	400842	13	NULL	NULL	0	NULL	histological analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this chapter we discuss study protocols aimed at integrating in vitro preparation of cells , small animal surgery , behavioral testing batteries , and histological analysis .
	manualset3
96920	1	400843	13	NULL	NULL	0	NULL	cluster	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this cluster , co-presence of bbp with the cna gene encoding collagen adhesin was a pattern consistently observed .
	manualset3
96921	2	400843	13	NULL	NULL	NULL	NULL	co-presence	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this cluster , co-presence of bbp with the cna gene encoding collagen adhesin was a pattern consistently observed .
	manualset3
96922	3	400843	13	NULL	NULL	0	NULL	bbp 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In this cluster , co-presence of bbp with the cna gene encoding collagen adhesin was a pattern consistently observed .
	manualset3
96923	4	400843	13	NULL	NULL	0	NULL	collagen adhesin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this cluster , co-presence of bbp with the cna gene encoding collagen adhesin was a pattern consistently observed .
	manualset3
96924	5	400843	13	NULL	NULL	0	NULL	cna gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In this cluster , co-presence of bbp with the cna gene encoding collagen adhesin was a pattern consistently observed .
	manualset3
96925	6	400843	13	NULL	NULL	0	NULL	pattern	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this cluster , co-presence of bbp with the cna gene encoding collagen adhesin was a pattern consistently observed .
	manualset3
96926	1	400844	13	NULL	NULL	0	NULL	communication	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this communication , an update on the epidemiology , prevalence and mechanisms of carbapenem-resistant Enterobacteriaceae in Lebanon and the surrounding region will be addressed in addition to the detection methods and required infection control practices .
	manualset3
96927	2	400844	13	NULL	NULL	0	NULL	epidemiology 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this communication , an update on the epidemiology , prevalence and mechanisms of carbapenem-resistant Enterobacteriaceae in Lebanon and the surrounding region will be addressed in addition to the detection methods and required infection control practices .
	manualset3
96928	3	400844	13	NULL	NULL	0	NULL	 prevalence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this communication , an update on the epidemiology , prevalence and mechanisms of carbapenem-resistant Enterobacteriaceae in Lebanon and the surrounding region will be addressed in addition to the detection methods and required infection control practices .
	manualset3
96929	4	400844	13	NULL	NULL	NULL	NULL	mechanisms	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this communication , an update on the epidemiology , prevalence and mechanisms of carbapenem-resistant Enterobacteriaceae in Lebanon and the surrounding region will be addressed in addition to the detection methods and required infection control practices .
	manualset3
96930	5	400844	13	NULL	NULL	0	NULL	carbapenem-resistant Enterobacteriaceae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this communication , an update on the epidemiology , prevalence and mechanisms of carbapenem-resistant Enterobacteriaceae in Lebanon and the surrounding region will be addressed in addition to the detection methods and required infection control practices .
	manualset3
96931	6	400844	13	NULL	NULL	0	NULL	Lebanon	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this communication , an update on the epidemiology , prevalence and mechanisms of carbapenem-resistant Enterobacteriaceae in Lebanon and the surrounding region will be addressed in addition to the detection methods and required infection control practices .
	manualset3
96932	7	400844	13	NULL	NULL	0	NULL	region	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this communication , an update on the epidemiology , prevalence and mechanisms of carbapenem-resistant Enterobacteriaceae in Lebanon and the surrounding region will be addressed in addition to the detection methods and required infection control practices .
	manualset3
96933	8	400844	13	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this communication , an update on the epidemiology , prevalence and mechanisms of carbapenem-resistant Enterobacteriaceae in Lebanon and the surrounding region will be addressed in addition to the detection methods and required infection control practices .
	manualset3
96934	9	400844	13	NULL	NULL	0	NULL	detection methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this communication , an update on the epidemiology , prevalence and mechanisms of carbapenem-resistant Enterobacteriaceae in Lebanon and the surrounding region will be addressed in addition to the detection methods and required infection control practices .
	manualset3
96935	10	400844	13	NULL	NULL	0	NULL	infection control practices	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this communication , an update on the epidemiology , prevalence and mechanisms of carbapenem-resistant Enterobacteriaceae in Lebanon and the surrounding region will be addressed in addition to the detection methods and required infection control practices .
	manualset3
96936	1	400845	13	NULL	NULL	0	NULL	158	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	158 males employees in the metal industry , aged 35-44 years , were examined to determine the prevalence of tenderness and pain in the neck and shoulders .
	manualset3
96937	2	400845	13	NULL	NULL	0	NULL	males employees	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	158 males employees in the metal industry , aged 35-44 years , were examined to determine the prevalence of tenderness and pain in the neck and shoulders .
	manualset3
96938	3	400845	13	NULL	NULL	0	NULL	metal industry	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	158 males employees in the metal industry , aged 35-44 years , were examined to determine the prevalence of tenderness and pain in the neck and shoulders .
	manualset3
96939	4	400845	13	NULL	NULL	0	NULL	aged 35-44 years	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	158 males employees in the metal industry , aged 35-44 years , were examined to determine the prevalence of tenderness and pain in the neck and shoulders .
	manualset3
96940	5	400845	13	NULL	NULL	0	NULL	prevalence of tenderness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	158 males employees in the metal industry , aged 35-44 years , were examined to determine the prevalence of tenderness and pain in the neck and shoulders .
	manualset3
96941	6	400845	13	NULL	NULL	0	NULL	pain 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	158 males employees in the metal industry , aged 35-44 years , were examined to determine the prevalence of tenderness and pain in the neck and shoulders .
	manualset3
96942	7	400845	13	NULL	NULL	0	NULL	neck 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	158 males employees in the metal industry , aged 35-44 years , were examined to determine the prevalence of tenderness and pain in the neck and shoulders .
	manualset3
96943	8	400845	13	NULL	NULL	0	NULL	shoulders	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	158 males employees in the metal industry , aged 35-44 years , were examined to determine the prevalence of tenderness and pain in the neck and shoulders .
	manualset3
96944	1	400846	13	NULL	NULL	0	NULL	context	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this context total lymph node count is not a quality criterion because nodal yield is overly influenced by the individual patient 's anatomy , surgical technique , template applied and pathological work-up .
	manualset3
96945	2	400846	13	NULL	NULL	0	NULL	total lymph node count	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this context total lymph node count is not a quality criterion because nodal yield is overly influenced by the individual patient 's anatomy , surgical technique , template applied and pathological work-up .
	manualset3
96946	3	400846	13	NULL	NULL	0	NULL	 quality criterion	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this context total lymph node count is not a quality criterion because nodal yield is overly influenced by the individual patient 's anatomy , surgical technique , template applied and pathological work-up .
	manualset3
96947	4	400846	13	NULL	NULL	0	NULL	nodal yield	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this context total lymph node count is not a quality criterion because nodal yield is overly influenced by the individual patient 's anatomy , surgical technique , template applied and pathological work-up .
	manualset3
96948	5	400846	13	NULL	NULL	0	NULL	individual patient 's anatomy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this context total lymph node count is not a quality criterion because nodal yield is overly influenced by the individual patient 's anatomy , surgical technique , template applied and pathological work-up .
	manualset3
96949	6	400846	13	NULL	NULL	0	NULL	surgical technique	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this context total lymph node count is not a quality criterion because nodal yield is overly influenced by the individual patient 's anatomy , surgical technique , template applied and pathological work-up .
	manualset3
96950	7	400846	13	NULL	NULL	0	NULL	 template	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this context total lymph node count is not a quality criterion because nodal yield is overly influenced by the individual patient 's anatomy , surgical technique , template applied and pathological work-up .
	manualset3
96951	8	400846	13	NULL	NULL	0	NULL	pathological work-up	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this context total lymph node count is not a quality criterion because nodal yield is overly influenced by the individual patient 's anatomy , surgical technique , template applied and pathological work-up .
	manualset3
96952	1	400847	13	NULL	NULL	0	NULL	context	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this context , treatment with PHA-767491 abolished DNA synthesis by inhibiting Cdc7 but is less effective in triggering cell death , although Mcl-1 protein is no longer detectable .
	manualset3
96953	2	400847	13	NULL	NULL	0	NULL	treatment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this context , treatment with PHA-767491 abolished DNA synthesis by inhibiting Cdc7 but is less effective in triggering cell death , although Mcl-1 protein is no longer detectable .
	manualset3
96954	3	400847	13	NULL	NULL	0	NULL	PHA-767491 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this context , treatment with PHA-767491 abolished DNA synthesis by inhibiting Cdc7 but is less effective in triggering cell death , although Mcl-1 protein is no longer detectable .
	manualset3
96955	4	400847	13	NULL	NULL	0	NULL	 DNA synthesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this context , treatment with PHA-767491 abolished DNA synthesis by inhibiting Cdc7 but is less effective in triggering cell death , although Mcl-1 protein is no longer detectable .
	manualset3
96956	5	400847	13	NULL	NULL	NULL	NULL	Cdc7	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this context , treatment with PHA-767491 abolished DNA synthesis by inhibiting Cdc7 but is less effective in triggering cell death , although Mcl-1 protein is no longer detectable .
	manualset3
96957	6	400847	13	NULL	NULL	0	NULL	cell death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this context , treatment with PHA-767491 abolished DNA synthesis by inhibiting Cdc7 but is less effective in triggering cell death , although Mcl-1 protein is no longer detectable .
	manualset3
96958	7	400847	13	NULL	NULL	0	NULL	Mcl-1 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this context , treatment with PHA-767491 abolished DNA synthesis by inhibiting Cdc7 but is less effective in triggering cell death , although Mcl-1 protein is no longer detectable .
	manualset3
96959	1	400848	13	NULL	NULL	0	NULL	context	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this context , we have undertaken functional analyses of ABCB1 polymorphisms .
	manualset3
96960	2	400848	13	NULL	NULL	0	NULL	functional analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this context , we have undertaken functional analyses of ABCB1 polymorphisms .
	manualset3
96961	3	400848	13	NULL	NULL	0	NULL	ABCB1 polymorphisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this context , we have undertaken functional analyses of ABCB1 polymorphisms .
	manualset3
96962	1	400849	13	NULL	NULL	0	NULL	contribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this contribution we provide an update of flavin-based BL sensors of the LOV and BLUF type , from prokaryotic microorganisms , with special emphasis to their light-activation pathways and molecular signal-transduction mechanisms .
	manualset3
96963	2	400849	13	NULL	NULL	NULL	NULL	flavin-based BL sensors	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this contribution we provide an update of flavin-based BL sensors of the LOV and BLUF type , from prokaryotic microorganisms , with special emphasis to their light-activation pathways and molecular signal-transduction mechanisms .
	manualset3
96964	3	400849	13	NULL	NULL	0	NULL	LOV type	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this contribution we provide an update of flavin-based BL sensors of the LOV and BLUF type , from prokaryotic microorganisms , with special emphasis to their light-activation pathways and molecular signal-transduction mechanisms .
	manualset3
96965	4	400849	13	NULL	NULL	0	NULL	BLUF type	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this contribution we provide an update of flavin-based BL sensors of the LOV and BLUF type , from prokaryotic microorganisms , with special emphasis to their light-activation pathways and molecular signal-transduction mechanisms .
	manualset3
96966	5	400849	13	NULL	NULL	0	NULL	prokaryotic microorganisms 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this contribution we provide an update of flavin-based BL sensors of the LOV and BLUF type , from prokaryotic microorganisms , with special emphasis to their light-activation pathways and molecular signal-transduction mechanisms .
	manualset3
96967	6	400849	13	NULL	NULL	0	NULL	emphasis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this contribution we provide an update of flavin-based BL sensors of the LOV and BLUF type , from prokaryotic microorganisms , with special emphasis to their light-activation pathways and molecular signal-transduction mechanisms .
	manualset3
96968	7	400849	13	NULL	NULL	0	NULL	light-activation pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this contribution we provide an update of flavin-based BL sensors of the LOV and BLUF type , from prokaryotic microorganisms , with special emphasis to their light-activation pathways and molecular signal-transduction mechanisms .
	manualset3
96969	8	400849	13	NULL	NULL	0	NULL	molecular signal-transduction mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this contribution we provide an update of flavin-based BL sensors of the LOV and BLUF type , from prokaryotic microorganisms , with special emphasis to their light-activation pathways and molecular signal-transduction mechanisms .
	manualset3
96970	1	400850	13	NULL	NULL	0	NULL	epidemiological study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this epidemiological study , we examined whether plasma phospholipids can be used for accurate biological monitoring of the LCPUFA state or whether analysis of erythrocyte membrane phospholipids is indispensable .
	manualset3
96971	2	400850	13	NULL	NULL	0	NULL	plasma phospholipids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this epidemiological study , we examined whether plasma phospholipids can be used for accurate biological monitoring of the LCPUFA state or whether analysis of erythrocyte membrane phospholipids is indispensable .
	manualset3
96972	3	400850	13	NULL	NULL	0	NULL	biological monitoring	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this epidemiological study , we examined whether plasma phospholipids can be used for accurate biological monitoring of the LCPUFA state or whether analysis of erythrocyte membrane phospholipids is indispensable .
	manualset3
96973	4	400850	13	NULL	NULL	0	NULL	LCPUFA state	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this epidemiological study , we examined whether plasma phospholipids can be used for accurate biological monitoring of the LCPUFA state or whether analysis of erythrocyte membrane phospholipids is indispensable .
	manualset3
96974	5	400850	13	NULL	NULL	0	NULL	analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this epidemiological study , we examined whether plasma phospholipids can be used for accurate biological monitoring of the LCPUFA state or whether analysis of erythrocyte membrane phospholipids is indispensable .
	manualset3
96975	6	400850	13	NULL	NULL	0	NULL	erythrocyte membrane phospholipids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this epidemiological study , we examined whether plasma phospholipids can be used for accurate biological monitoring of the LCPUFA state or whether analysis of erythrocyte membrane phospholipids is indispensable .
	manualset3
96976	1	400851	13	NULL	NULL	0	NULL	follow-up study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this follow-up study , we demonstrate that : 1 ) OPN gene transcription is regulated by a constitutive transcriptional repressor protein , heterogeneous nuclear ribonucleoprotein A/B ( hnRNP A/B ) ; 2 ) inhibition of in vivo hnRNP DNA binding activity is accompanied by increased S-nitrosylation of hnRNP A/B in the setting of lipopolysaccharide ( LPS ) - mediated NO synthesis ; 3 ) inhibition of LPS mediated NO synthesis restores hnRNP DNA binding and decreases the extent of S-nitrosylation ; and 4 ) S-nitrosylation of hnRNP at cysteine 104 inhibits in vitro DNA binding activity , which is reversed by dithiothreitol .
	manualset3
96977	2	400851	13	NULL	NULL	0	NULL	OPN gene transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this follow-up study , we demonstrate that : 1 ) OPN gene transcription is regulated by a constitutive transcriptional repressor protein , heterogeneous nuclear ribonucleoprotein A/B ( hnRNP A/B ) ; 2 ) inhibition of in vivo hnRNP DNA binding activity is accompanied by increased S-nitrosylation of hnRNP A/B in the setting of lipopolysaccharide ( LPS ) - mediated NO synthesis ; 3 ) inhibition of LPS mediated NO synthesis restores hnRNP DNA binding and decreases the extent of S-nitrosylation ; and 4 ) S-nitrosylation of hnRNP at cysteine 104 inhibits in vitro DNA binding activity , which is reversed by dithiothreitol .
	manualset3
96978	3	400851	13	NULL	NULL	0	NULL	constitutive transcriptional repressor protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this follow-up study , we demonstrate that : 1 ) OPN gene transcription is regulated by a constitutive transcriptional repressor protein , heterogeneous nuclear ribonucleoprotein A/B ( hnRNP A/B ) ; 2 ) inhibition of in vivo hnRNP DNA binding activity is accompanied by increased S-nitrosylation of hnRNP A/B in the setting of lipopolysaccharide ( LPS ) - mediated NO synthesis ; 3 ) inhibition of LPS mediated NO synthesis restores hnRNP DNA binding and decreases the extent of S-nitrosylation ; and 4 ) S-nitrosylation of hnRNP at cysteine 104 inhibits in vitro DNA binding activity , which is reversed by dithiothreitol .
	manualset3
96979	4	400851	13	NULL	NULL	0	NULL	heterogeneous nuclear ribonucleoprotein A/B ( hnRNP A/B )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this follow-up study , we demonstrate that : 1 ) OPN gene transcription is regulated by a constitutive transcriptional repressor protein , heterogeneous nuclear ribonucleoprotein A/B ( hnRNP A/B ) ; 2 ) inhibition of in vivo hnRNP DNA binding activity is accompanied by increased S-nitrosylation of hnRNP A/B in the setting of lipopolysaccharide ( LPS ) - mediated NO synthesis ; 3 ) inhibition of LPS mediated NO synthesis restores hnRNP DNA binding and decreases the extent of S-nitrosylation ; and 4 ) S-nitrosylation of hnRNP at cysteine 104 inhibits in vitro DNA binding activity , which is reversed by dithiothreitol .
	manualset3
96980	5	400851	13	NULL	NULL	0	NULL	 inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this follow-up study , we demonstrate that : 1 ) OPN gene transcription is regulated by a constitutive transcriptional repressor protein , heterogeneous nuclear ribonucleoprotein A/B ( hnRNP A/B ) ; 2 ) inhibition of in vivo hnRNP DNA binding activity is accompanied by increased S-nitrosylation of hnRNP A/B in the setting of lipopolysaccharide ( LPS ) - mediated NO synthesis ; 3 ) inhibition of LPS mediated NO synthesis restores hnRNP DNA binding and decreases the extent of S-nitrosylation ; and 4 ) S-nitrosylation of hnRNP at cysteine 104 inhibits in vitro DNA binding activity , which is reversed by dithiothreitol .
	manualset3
96981	6	400851	13	NULL	NULL	0	NULL	 in vivo hnRNP DNA binding activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this follow-up study , we demonstrate that : 1 ) OPN gene transcription is regulated by a constitutive transcriptional repressor protein , heterogeneous nuclear ribonucleoprotein A/B ( hnRNP A/B ) ; 2 ) inhibition of in vivo hnRNP DNA binding activity is accompanied by increased S-nitrosylation of hnRNP A/B in the setting of lipopolysaccharide ( LPS ) - mediated NO synthesis ; 3 ) inhibition of LPS mediated NO synthesis restores hnRNP DNA binding and decreases the extent of S-nitrosylation ; and 4 ) S-nitrosylation of hnRNP at cysteine 104 inhibits in vitro DNA binding activity , which is reversed by dithiothreitol .
	manualset3
96982	7	400851	13	NULL	NULL	0	NULL	S-nitrosylation of hnRNP A/B	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this follow-up study , we demonstrate that : 1 ) OPN gene transcription is regulated by a constitutive transcriptional repressor protein , heterogeneous nuclear ribonucleoprotein A/B ( hnRNP A/B ) ; 2 ) inhibition of in vivo hnRNP DNA binding activity is accompanied by increased S-nitrosylation of hnRNP A/B in the setting of lipopolysaccharide ( LPS ) - mediated NO synthesis ; 3 ) inhibition of LPS mediated NO synthesis restores hnRNP DNA binding and decreases the extent of S-nitrosylation ; and 4 ) S-nitrosylation of hnRNP at cysteine 104 inhibits in vitro DNA binding activity , which is reversed by dithiothreitol .
	manualset3
96983	8	400851	13	NULL	NULL	0	NULL	lipopolysaccharide ( LPS )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In this follow-up study , we demonstrate that : 1 ) OPN gene transcription is regulated by a constitutive transcriptional repressor protein , heterogeneous nuclear ribonucleoprotein A/B ( hnRNP A/B ) ; 2 ) inhibition of in vivo hnRNP DNA binding activity is accompanied by increased S-nitrosylation of hnRNP A/B in the setting of lipopolysaccharide ( LPS ) - mediated NO synthesis ; 3 ) inhibition of LPS mediated NO synthesis restores hnRNP DNA binding and decreases the extent of S-nitrosylation ; and 4 ) S-nitrosylation of hnRNP at cysteine 104 inhibits in vitro DNA binding activity , which is reversed by dithiothreitol .
	manualset3
96984	9	400851	13	NULL	NULL	0	NULL	NO synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this follow-up study , we demonstrate that : 1 ) OPN gene transcription is regulated by a constitutive transcriptional repressor protein , heterogeneous nuclear ribonucleoprotein A/B ( hnRNP A/B ) ; 2 ) inhibition of in vivo hnRNP DNA binding activity is accompanied by increased S-nitrosylation of hnRNP A/B in the setting of lipopolysaccharide ( LPS ) - mediated NO synthesis ; 3 ) inhibition of LPS mediated NO synthesis restores hnRNP DNA binding and decreases the extent of S-nitrosylation ; and 4 ) S-nitrosylation of hnRNP at cysteine 104 inhibits in vitro DNA binding activity , which is reversed by dithiothreitol .
	manualset3
96985	10	400851	13	NULL	NULL	0	NULL	inhibition 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this follow-up study , we demonstrate that : 1 ) OPN gene transcription is regulated by a constitutive transcriptional repressor protein , heterogeneous nuclear ribonucleoprotein A/B ( hnRNP A/B ) ; 2 ) inhibition of in vivo hnRNP DNA binding activity is accompanied by increased S-nitrosylation of hnRNP A/B in the setting of lipopolysaccharide ( LPS ) - mediated NO synthesis ; 3 ) inhibition of LPS mediated NO synthesis restores hnRNP DNA binding and decreases the extent of S-nitrosylation ; and 4 ) S-nitrosylation of hnRNP at cysteine 104 inhibits in vitro DNA binding activity , which is reversed by dithiothreitol .
	manualset3
96986	11	400851	13	NULL	NULL	0	NULL	LPS	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In this follow-up study , we demonstrate that : 1 ) OPN gene transcription is regulated by a constitutive transcriptional repressor protein , heterogeneous nuclear ribonucleoprotein A/B ( hnRNP A/B ) ; 2 ) inhibition of in vivo hnRNP DNA binding activity is accompanied by increased S-nitrosylation of hnRNP A/B in the setting of lipopolysaccharide ( LPS ) - mediated NO synthesis ; 3 ) inhibition of LPS mediated NO synthesis restores hnRNP DNA binding and decreases the extent of S-nitrosylation ; and 4 ) S-nitrosylation of hnRNP at cysteine 104 inhibits in vitro DNA binding activity , which is reversed by dithiothreitol .
	manualset3
96987	12	400851	13	NULL	NULL	0	NULL	NO synthesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this follow-up study , we demonstrate that : 1 ) OPN gene transcription is regulated by a constitutive transcriptional repressor protein , heterogeneous nuclear ribonucleoprotein A/B ( hnRNP A/B ) ; 2 ) inhibition of in vivo hnRNP DNA binding activity is accompanied by increased S-nitrosylation of hnRNP A/B in the setting of lipopolysaccharide ( LPS ) - mediated NO synthesis ; 3 ) inhibition of LPS mediated NO synthesis restores hnRNP DNA binding and decreases the extent of S-nitrosylation ; and 4 ) S-nitrosylation of hnRNP at cysteine 104 inhibits in vitro DNA binding activity , which is reversed by dithiothreitol .
	manualset3
96988	13	400851	13	NULL	NULL	0	NULL	restores 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this follow-up study , we demonstrate that : 1 ) OPN gene transcription is regulated by a constitutive transcriptional repressor protein , heterogeneous nuclear ribonucleoprotein A/B ( hnRNP A/B ) ; 2 ) inhibition of in vivo hnRNP DNA binding activity is accompanied by increased S-nitrosylation of hnRNP A/B in the setting of lipopolysaccharide ( LPS ) - mediated NO synthesis ; 3 ) inhibition of LPS mediated NO synthesis restores hnRNP DNA binding and decreases the extent of S-nitrosylation ; and 4 ) S-nitrosylation of hnRNP at cysteine 104 inhibits in vitro DNA binding activity , which is reversed by dithiothreitol .
	manualset3
96989	14	400851	13	NULL	NULL	0	NULL	hnRNP DNA binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this follow-up study , we demonstrate that : 1 ) OPN gene transcription is regulated by a constitutive transcriptional repressor protein , heterogeneous nuclear ribonucleoprotein A/B ( hnRNP A/B ) ; 2 ) inhibition of in vivo hnRNP DNA binding activity is accompanied by increased S-nitrosylation of hnRNP A/B in the setting of lipopolysaccharide ( LPS ) - mediated NO synthesis ; 3 ) inhibition of LPS mediated NO synthesis restores hnRNP DNA binding and decreases the extent of S-nitrosylation ; and 4 ) S-nitrosylation of hnRNP at cysteine 104 inhibits in vitro DNA binding activity , which is reversed by dithiothreitol .
	manualset3
96990	15	400851	13	NULL	NULL	0	NULL	 extent of S-nitrosylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this follow-up study , we demonstrate that : 1 ) OPN gene transcription is regulated by a constitutive transcriptional repressor protein , heterogeneous nuclear ribonucleoprotein A/B ( hnRNP A/B ) ; 2 ) inhibition of in vivo hnRNP DNA binding activity is accompanied by increased S-nitrosylation of hnRNP A/B in the setting of lipopolysaccharide ( LPS ) - mediated NO synthesis ; 3 ) inhibition of LPS mediated NO synthesis restores hnRNP DNA binding and decreases the extent of S-nitrosylation ; and 4 ) S-nitrosylation of hnRNP at cysteine 104 inhibits in vitro DNA binding activity , which is reversed by dithiothreitol .
	manualset3
96991	16	400851	13	NULL	NULL	0	NULL	S-nitrosylation of hnRNP 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this follow-up study , we demonstrate that : 1 ) OPN gene transcription is regulated by a constitutive transcriptional repressor protein , heterogeneous nuclear ribonucleoprotein A/B ( hnRNP A/B ) ; 2 ) inhibition of in vivo hnRNP DNA binding activity is accompanied by increased S-nitrosylation of hnRNP A/B in the setting of lipopolysaccharide ( LPS ) - mediated NO synthesis ; 3 ) inhibition of LPS mediated NO synthesis restores hnRNP DNA binding and decreases the extent of S-nitrosylation ; and 4 ) S-nitrosylation of hnRNP at cysteine 104 inhibits in vitro DNA binding activity , which is reversed by dithiothreitol .
	manualset3
96992	17	400851	13	NULL	NULL	0	NULL	cysteine 104	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this follow-up study , we demonstrate that : 1 ) OPN gene transcription is regulated by a constitutive transcriptional repressor protein , heterogeneous nuclear ribonucleoprotein A/B ( hnRNP A/B ) ; 2 ) inhibition of in vivo hnRNP DNA binding activity is accompanied by increased S-nitrosylation of hnRNP A/B in the setting of lipopolysaccharide ( LPS ) - mediated NO synthesis ; 3 ) inhibition of LPS mediated NO synthesis restores hnRNP DNA binding and decreases the extent of S-nitrosylation ; and 4 ) S-nitrosylation of hnRNP at cysteine 104 inhibits in vitro DNA binding activity , which is reversed by dithiothreitol .
	manualset3
96993	18	400851	13	NULL	NULL	0	NULL	in vitro DNA binding activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this follow-up study , we demonstrate that : 1 ) OPN gene transcription is regulated by a constitutive transcriptional repressor protein , heterogeneous nuclear ribonucleoprotein A/B ( hnRNP A/B ) ; 2 ) inhibition of in vivo hnRNP DNA binding activity is accompanied by increased S-nitrosylation of hnRNP A/B in the setting of lipopolysaccharide ( LPS ) - mediated NO synthesis ; 3 ) inhibition of LPS mediated NO synthesis restores hnRNP DNA binding and decreases the extent of S-nitrosylation ; and 4 ) S-nitrosylation of hnRNP at cysteine 104 inhibits in vitro DNA binding activity , which is reversed by dithiothreitol .
	manualset3
96994	19	400851	13	NULL	NULL	0	NULL	dithiothreitol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this follow-up study , we demonstrate that : 1 ) OPN gene transcription is regulated by a constitutive transcriptional repressor protein , heterogeneous nuclear ribonucleoprotein A/B ( hnRNP A/B ) ; 2 ) inhibition of in vivo hnRNP DNA binding activity is accompanied by increased S-nitrosylation of hnRNP A/B in the setting of lipopolysaccharide ( LPS ) - mediated NO synthesis ; 3 ) inhibition of LPS mediated NO synthesis restores hnRNP DNA binding and decreases the extent of S-nitrosylation ; and 4 ) S-nitrosylation of hnRNP at cysteine 104 inhibits in vitro DNA binding activity , which is reversed by dithiothreitol .
	manualset3
96995	1	400852	13	NULL	NULL	NULL	NULL	mechanism	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this mechanism , the rate constant of the reaction would be directly related with the strength of the nucleophilic attack of the C-1 hydroxyl group , which depends on the chemical shift of the carbon C-1 ( delta ( 1 ) ) obtained by ( 13 ) C-NMR .
	manualset3
96996	2	400852	13	NULL	NULL	0	NULL	rate constant 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this mechanism , the rate constant of the reaction would be directly related with the strength of the nucleophilic attack of the C-1 hydroxyl group , which depends on the chemical shift of the carbon C-1 ( delta ( 1 ) ) obtained by ( 13 ) C-NMR .
	manualset3
96997	3	400852	13	NULL	NULL	NULL	NULL	reaction	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this mechanism , the rate constant of the reaction would be directly related with the strength of the nucleophilic attack of the C-1 hydroxyl group , which depends on the chemical shift of the carbon C-1 ( delta ( 1 ) ) obtained by ( 13 ) C-NMR .
	manualset3
96998	4	400852	13	NULL	NULL	0	NULL	strength	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this mechanism , the rate constant of the reaction would be directly related with the strength of the nucleophilic attack of the C-1 hydroxyl group , which depends on the chemical shift of the carbon C-1 ( delta ( 1 ) ) obtained by ( 13 ) C-NMR .
	manualset3
96999	5	400852	13	NULL	NULL	0	NULL	nucleophilic attack	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this mechanism , the rate constant of the reaction would be directly related with the strength of the nucleophilic attack of the C-1 hydroxyl group , which depends on the chemical shift of the carbon C-1 ( delta ( 1 ) ) obtained by ( 13 ) C-NMR .
	manualset3
97000	6	400852	13	NULL	NULL	0	NULL	C-1 hydroxyl group	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this mechanism , the rate constant of the reaction would be directly related with the strength of the nucleophilic attack of the C-1 hydroxyl group , which depends on the chemical shift of the carbon C-1 ( delta ( 1 ) ) obtained by ( 13 ) C-NMR .
	manualset3
97001	7	400852	13	NULL	NULL	0	NULL	chemical shift	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this mechanism , the rate constant of the reaction would be directly related with the strength of the nucleophilic attack of the C-1 hydroxyl group , which depends on the chemical shift of the carbon C-1 ( delta ( 1 ) ) obtained by ( 13 ) C-NMR .
	manualset3
97002	8	400852	13	NULL	NULL	0	NULL	carbon C-1 ( delta ( 1 ) ) 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	In this mechanism , the rate constant of the reaction would be directly related with the strength of the nucleophilic attack of the C-1 hydroxyl group , which depends on the chemical shift of the carbon C-1 ( delta ( 1 ) ) obtained by ( 13 ) C-NMR .
	manualset3
97003	9	400852	13	NULL	NULL	0	NULL	C-NMR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this mechanism , the rate constant of the reaction would be directly related with the strength of the nucleophilic attack of the C-1 hydroxyl group , which depends on the chemical shift of the carbon C-1 ( delta ( 1 ) ) obtained by ( 13 ) C-NMR .
	manualset3
97004	1	400853	13	NULL	NULL	0	NULL	15d-PGJ ( 2 )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	15d-PGJ ( 2 ) inhibited expression of VEGFR-1 and VEGFR-2 receptors both at mRNA and protein levels .
	manualset3
97005	2	400853	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	15d-PGJ ( 2 ) inhibited expression of VEGFR-1 and VEGFR-2 receptors both at mRNA and protein levels .
	manualset3
97006	3	400853	13	NULL	NULL	0	NULL	VEGFR-1 receptors  	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	15d-PGJ ( 2 ) inhibited expression of VEGFR-1 and VEGFR-2 receptors both at mRNA and protein levels .
	manualset3
97007	4	400853	13	NULL	NULL	0	NULL	VEGFR-2 receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	15d-PGJ ( 2 ) inhibited expression of VEGFR-1 and VEGFR-2 receptors both at mRNA and protein levels .
	manualset3
97008	5	400853	13	NULL	NULL	0	NULL	mRNA levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	15d-PGJ ( 2 ) inhibited expression of VEGFR-1 and VEGFR-2 receptors both at mRNA and protein levels .
	manualset3
97009	6	400853	13	NULL	NULL	0	NULL	protein levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	15d-PGJ ( 2 ) inhibited expression of VEGFR-1 and VEGFR-2 receptors both at mRNA and protein levels .
	manualset3
97010	1	400854	13	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this model neural representations of pitch height are primed by the location and pattern of excitation across auditory filter channels in relation to long-term memory templates for common stimuli .
	manualset3
97011	2	400854	13	NULL	NULL	0	NULL	neural representations of pitch height	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this model neural representations of pitch height are primed by the location and pattern of excitation across auditory filter channels in relation to long-term memory templates for common stimuli .
	manualset3
97012	3	400854	13	NULL	NULL	0	NULL	location of excitation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this model neural representations of pitch height are primed by the location and pattern of excitation across auditory filter channels in relation to long-term memory templates for common stimuli .
	manualset3
97013	4	400854	13	NULL	NULL	0	NULL	pattern of excitation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this model neural representations of pitch height are primed by the location and pattern of excitation across auditory filter channels in relation to long-term memory templates for common stimuli .
	manualset3
97014	5	400854	13	NULL	NULL	0	NULL	auditory filter channels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this model neural representations of pitch height are primed by the location and pattern of excitation across auditory filter channels in relation to long-term memory templates for common stimuli .
	manualset3
97015	6	400854	13	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In this model neural representations of pitch height are primed by the location and pattern of excitation across auditory filter channels in relation to long-term memory templates for common stimuli .
	manualset3
97016	7	400854	13	NULL	NULL	0	NULL	long-term memory	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this model neural representations of pitch height are primed by the location and pattern of excitation across auditory filter channels in relation to long-term memory templates for common stimuli .
	manualset3
97017	8	400854	13	NULL	NULL	0	NULL	common stimuli	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this model neural representations of pitch height are primed by the location and pattern of excitation across auditory filter channels in relation to long-term memory templates for common stimuli .
	manualset3
97018	1	400855	13	NULL	NULL	0	NULL	thrombosis model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this new thrombosis model induced by free radicals antithrombotic drugs ( aspirin , 200 mg/Kg , heparin , 2 mg/Kg ) and antioxidants ( vitamin C , 10 and 20 mg/Kg , allopurinol , 200 and 300 mg/Kg , vitamin E , 500 and 1000 mg/Kg ) have been tested .
	manualset3
97019	2	400855	13	NULL	NULL	0	NULL	free radicals antithrombotic drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In this new thrombosis model induced by free radicals antithrombotic drugs ( aspirin , 200 mg/Kg , heparin , 2 mg/Kg ) and antioxidants ( vitamin C , 10 and 20 mg/Kg , allopurinol , 200 and 300 mg/Kg , vitamin E , 500 and 1000 mg/Kg ) have been tested .
	manualset3
97020	3	400855	13	NULL	NULL	0	NULL	aspirin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In this new thrombosis model induced by free radicals antithrombotic drugs ( aspirin , 200 mg/Kg , heparin , 2 mg/Kg ) and antioxidants ( vitamin C , 10 and 20 mg/Kg , allopurinol , 200 and 300 mg/Kg , vitamin E , 500 and 1000 mg/Kg ) have been tested .
	manualset3
97021	4	400855	13	NULL	NULL	0	NULL	200 mg/Kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this new thrombosis model induced by free radicals antithrombotic drugs ( aspirin , 200 mg/Kg , heparin , 2 mg/Kg ) and antioxidants ( vitamin C , 10 and 20 mg/Kg , allopurinol , 200 and 300 mg/Kg , vitamin E , 500 and 1000 mg/Kg ) have been tested .
	manualset3
97022	5	400855	13	NULL	NULL	0	NULL	heparin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In this new thrombosis model induced by free radicals antithrombotic drugs ( aspirin , 200 mg/Kg , heparin , 2 mg/Kg ) and antioxidants ( vitamin C , 10 and 20 mg/Kg , allopurinol , 200 and 300 mg/Kg , vitamin E , 500 and 1000 mg/Kg ) have been tested .
	manualset3
97023	6	400855	13	NULL	NULL	0	NULL	2 mg/Kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this new thrombosis model induced by free radicals antithrombotic drugs ( aspirin , 200 mg/Kg , heparin , 2 mg/Kg ) and antioxidants ( vitamin C , 10 and 20 mg/Kg , allopurinol , 200 and 300 mg/Kg , vitamin E , 500 and 1000 mg/Kg ) have been tested .
	manualset3
97024	7	400855	13	NULL	NULL	NULL	NULL	antioxidants	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this new thrombosis model induced by free radicals antithrombotic drugs ( aspirin , 200 mg/Kg , heparin , 2 mg/Kg ) and antioxidants ( vitamin C , 10 and 20 mg/Kg , allopurinol , 200 and 300 mg/Kg , vitamin E , 500 and 1000 mg/Kg ) have been tested .
	manualset3
97025	8	400855	13	NULL	NULL	0	NULL	vitamin C	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this new thrombosis model induced by free radicals antithrombotic drugs ( aspirin , 200 mg/Kg , heparin , 2 mg/Kg ) and antioxidants ( vitamin C , 10 and 20 mg/Kg , allopurinol , 200 and 300 mg/Kg , vitamin E , 500 and 1000 mg/Kg ) have been tested .
	manualset3
97026	9	400855	13	NULL	NULL	0	NULL	10 mg/Kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this new thrombosis model induced by free radicals antithrombotic drugs ( aspirin , 200 mg/Kg , heparin , 2 mg/Kg ) and antioxidants ( vitamin C , 10 and 20 mg/Kg , allopurinol , 200 and 300 mg/Kg , vitamin E , 500 and 1000 mg/Kg ) have been tested .
	manualset3
97027	10	400855	13	NULL	NULL	0	NULL	20 mg/Kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this new thrombosis model induced by free radicals antithrombotic drugs ( aspirin , 200 mg/Kg , heparin , 2 mg/Kg ) and antioxidants ( vitamin C , 10 and 20 mg/Kg , allopurinol , 200 and 300 mg/Kg , vitamin E , 500 and 1000 mg/Kg ) have been tested .
	manualset3
97028	11	400855	13	NULL	NULL	0	NULL	allopurinol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In this new thrombosis model induced by free radicals antithrombotic drugs ( aspirin , 200 mg/Kg , heparin , 2 mg/Kg ) and antioxidants ( vitamin C , 10 and 20 mg/Kg , allopurinol , 200 and 300 mg/Kg , vitamin E , 500 and 1000 mg/Kg ) have been tested .
	manualset3
97029	12	400855	13	NULL	NULL	0	NULL	200 mg/Kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this new thrombosis model induced by free radicals antithrombotic drugs ( aspirin , 200 mg/Kg , heparin , 2 mg/Kg ) and antioxidants ( vitamin C , 10 and 20 mg/Kg , allopurinol , 200 and 300 mg/Kg , vitamin E , 500 and 1000 mg/Kg ) have been tested .
	manualset3
97030	13	400855	13	NULL	NULL	0	NULL	300 mg/Kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this new thrombosis model induced by free radicals antithrombotic drugs ( aspirin , 200 mg/Kg , heparin , 2 mg/Kg ) and antioxidants ( vitamin C , 10 and 20 mg/Kg , allopurinol , 200 and 300 mg/Kg , vitamin E , 500 and 1000 mg/Kg ) have been tested .
	manualset3
97031	14	400855	13	NULL	NULL	0	NULL	vitamin E	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this new thrombosis model induced by free radicals antithrombotic drugs ( aspirin , 200 mg/Kg , heparin , 2 mg/Kg ) and antioxidants ( vitamin C , 10 and 20 mg/Kg , allopurinol , 200 and 300 mg/Kg , vitamin E , 500 and 1000 mg/Kg ) have been tested .
	manualset3
97032	15	400855	13	NULL	NULL	0	NULL	500 mg/Kg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this new thrombosis model induced by free radicals antithrombotic drugs ( aspirin , 200 mg/Kg , heparin , 2 mg/Kg ) and antioxidants ( vitamin C , 10 and 20 mg/Kg , allopurinol , 200 and 300 mg/Kg , vitamin E , 500 and 1000 mg/Kg ) have been tested .
	manualset3
97033	16	400855	13	NULL	NULL	0	NULL	1000 mg/Kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this new thrombosis model induced by free radicals antithrombotic drugs ( aspirin , 200 mg/Kg , heparin , 2 mg/Kg ) and antioxidants ( vitamin C , 10 and 20 mg/Kg , allopurinol , 200 and 300 mg/Kg , vitamin E , 500 and 1000 mg/Kg ) have been tested .
	manualset3
97034	1	400856	13	NULL	NULL	0	NULL	overview	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this overview , a selection of cage-type receptors is presented whose inner cavity is functionalized with groups that can engage in directed interactions with an included guest .
	manualset3
97035	2	400856	13	NULL	NULL	0	NULL	selection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this overview , a selection of cage-type receptors is presented whose inner cavity is functionalized with groups that can engage in directed interactions with an included guest .
	manualset3
97037	4	400856	13	NULL	NULL	NULL	NULL	cage-type receptors	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this overview , a selection of cage-type receptors is presented whose inner cavity is functionalized with groups that can engage in directed interactions with an included guest .
	manualset3
97038	5	400856	13	NULL	NULL	NULL	NULL	 inner cavity	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this overview , a selection of cage-type receptors is presented whose inner cavity is functionalized with groups that can engage in directed interactions with an included guest .
	manualset3
97039	6	400856	13	NULL	NULL	0	NULL	 groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this overview , a selection of cage-type receptors is presented whose inner cavity is functionalized with groups that can engage in directed interactions with an included guest .
	manualset3
97040	7	400856	13	NULL	NULL	0	NULL	interactions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this overview , a selection of cage-type receptors is presented whose inner cavity is functionalized with groups that can engage in directed interactions with an included guest .
	manualset3
97041	8	400856	13	NULL	NULL	0	NULL	 guest	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this overview , a selection of cage-type receptors is presented whose inner cavity is functionalized with groups that can engage in directed interactions with an included guest .
	manualset3
97042	1	400857	13	NULL	NULL	0	NULL	 paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , alpha-tricalcium phosphate ( alpha-TCP ) and tetracalcium phosphate ( TTCP ) respectively were chosen as basic compositions of phosphate bone cements .
	manualset3
97043	2	400857	13	NULL	NULL	0	NULL	alpha-tricalcium phosphate ( alpha-TCP ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , alpha-tricalcium phosphate ( alpha-TCP ) and tetracalcium phosphate ( TTCP ) respectively were chosen as basic compositions of phosphate bone cements .
	manualset3
97044	3	400857	13	NULL	NULL	0	NULL	tetracalcium phosphate ( TTCP )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , alpha-tricalcium phosphate ( alpha-TCP ) and tetracalcium phosphate ( TTCP ) respectively were chosen as basic compositions of phosphate bone cements .
	manualset3
97045	4	400857	13	NULL	NULL	0	NULL	compositions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , alpha-tricalcium phosphate ( alpha-TCP ) and tetracalcium phosphate ( TTCP ) respectively were chosen as basic compositions of phosphate bone cements .
	manualset3
97046	5	400857	13	NULL	NULL	0	NULL	phosphate bone cements	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , alpha-tricalcium phosphate ( alpha-TCP ) and tetracalcium phosphate ( TTCP ) respectively were chosen as basic compositions of phosphate bone cements .
	manualset3
97047	1	400858	13	NULL	NULL	0	NULL	paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , node repositioning and node addition are the two methods of mesh modification examined for coarse meshes .
	manualset3
97048	2	400858	13	NULL	NULL	0	NULL	node 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , node repositioning and node addition are the two methods of mesh modification examined for coarse meshes .
	manualset3
97049	3	400858	13	NULL	NULL	0	NULL	node addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , node repositioning and node addition are the two methods of mesh modification examined for coarse meshes .
	manualset3
97050	4	400858	13	NULL	NULL	0	NULL	two methods 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , node repositioning and node addition are the two methods of mesh modification examined for coarse meshes .
	manualset3
97051	5	400858	13	NULL	NULL	0	NULL	mesh modification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , node repositioning and node addition are the two methods of mesh modification examined for coarse meshes .
	manualset3
97052	6	400858	13	NULL	NULL	0	NULL	coarse meshes	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , node repositioning and node addition are the two methods of mesh modification examined for coarse meshes .
	manualset3
97053	1	400859	13	NULL	NULL	0	NULL	paper 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , the accumulation of surfactant on the surface of poly ( styrene-co-butyl acrylate ) latex is studied using Rutherford Backscattering ( RBS ) and compared with results from a model that is based on the diffusive transport of particles and surfactant .
	manualset3
97054	2	400859	13	NULL	NULL	NULL	NULL	accumulation of surfactant 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this paper , the accumulation of surfactant on the surface of poly ( styrene-co-butyl acrylate ) latex is studied using Rutherford Backscattering ( RBS ) and compared with results from a model that is based on the diffusive transport of particles and surfactant .
	manualset3
97055	3	400859	13	NULL	NULL	0	NULL	surface of poly ( styrene-co-butyl acrylate ) latex 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , the accumulation of surfactant on the surface of poly ( styrene-co-butyl acrylate ) latex is studied using Rutherford Backscattering ( RBS ) and compared with results from a model that is based on the diffusive transport of particles and surfactant .
	manualset3
97056	4	400859	13	NULL	NULL	0	NULL	Rutherford Backscattering ( RBS ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , the accumulation of surfactant on the surface of poly ( styrene-co-butyl acrylate ) latex is studied using Rutherford Backscattering ( RBS ) and compared with results from a model that is based on the diffusive transport of particles and surfactant .
	manualset3
97057	5	400859	13	NULL	NULL	0	NULL	results	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , the accumulation of surfactant on the surface of poly ( styrene-co-butyl acrylate ) latex is studied using Rutherford Backscattering ( RBS ) and compared with results from a model that is based on the diffusive transport of particles and surfactant .
	manualset3
97058	6	400859	13	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , the accumulation of surfactant on the surface of poly ( styrene-co-butyl acrylate ) latex is studied using Rutherford Backscattering ( RBS ) and compared with results from a model that is based on the diffusive transport of particles and surfactant .
	manualset3
97059	7	400859	13	NULL	NULL	0	NULL	transport of particles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , the accumulation of surfactant on the surface of poly ( styrene-co-butyl acrylate ) latex is studied using Rutherford Backscattering ( RBS ) and compared with results from a model that is based on the diffusive transport of particles and surfactant .
	manualset3
97060	8	400859	13	NULL	NULL	0	NULL	surfactant	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , the accumulation of surfactant on the surface of poly ( styrene-co-butyl acrylate ) latex is studied using Rutherford Backscattering ( RBS ) and compared with results from a model that is based on the diffusive transport of particles and surfactant .
	manualset3
97061	1	400860	13	NULL	NULL	0	NULL	 paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , the author lists the key elements comprising good veterinary governance and discusses the World Organisation for Animal Health ( OIE ) standards for the quality of VS. The OIE Tool for the Evaluation of the Performance of Veterinary Services ( OIE PVS Tool ) is introduced and its relevance in assessing compliance with OIE standards to prevent the spread of pathogens through trade is highlighted .
	manualset3
97062	2	400860	13	NULL	NULL	0	NULL	author	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , the author lists the key elements comprising good veterinary governance and discusses the World Organisation for Animal Health ( OIE ) standards for the quality of VS. The OIE Tool for the Evaluation of the Performance of Veterinary Services ( OIE PVS Tool ) is introduced and its relevance in assessing compliance with OIE standards to prevent the spread of pathogens through trade is highlighted .
	manualset3
97063	3	400860	13	NULL	NULL	0	NULL	key elements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , the author lists the key elements comprising good veterinary governance and discusses the World Organisation for Animal Health ( OIE ) standards for the quality of VS. The OIE Tool for the Evaluation of the Performance of Veterinary Services ( OIE PVS Tool ) is introduced and its relevance in assessing compliance with OIE standards to prevent the spread of pathogens through trade is highlighted .
	manualset3
97064	4	400860	13	NULL	NULL	0	NULL	veterinary governance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , the author lists the key elements comprising good veterinary governance and discusses the World Organisation for Animal Health ( OIE ) standards for the quality of VS. The OIE Tool for the Evaluation of the Performance of Veterinary Services ( OIE PVS Tool ) is introduced and its relevance in assessing compliance with OIE standards to prevent the spread of pathogens through trade is highlighted .
	manualset3
97065	5	400860	13	NULL	NULL	0	NULL	World Organisation for Animal Health ( OIE ) 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , the author lists the key elements comprising good veterinary governance and discusses the World Organisation for Animal Health ( OIE ) standards for the quality of VS. The OIE Tool for the Evaluation of the Performance of Veterinary Services ( OIE PVS Tool ) is introduced and its relevance in assessing compliance with OIE standards to prevent the spread of pathogens through trade is highlighted .
	manualset3
97066	6	400860	13	NULL	NULL	0	NULL	standards 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , the author lists the key elements comprising good veterinary governance and discusses the World Organisation for Animal Health ( OIE ) standards for the quality of VS. The OIE Tool for the Evaluation of the Performance of Veterinary Services ( OIE PVS Tool ) is introduced and its relevance in assessing compliance with OIE standards to prevent the spread of pathogens through trade is highlighted .
	manualset3
97067	7	400860	13	NULL	NULL	0	NULL	quality of VS	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , the author lists the key elements comprising good veterinary governance and discusses the World Organisation for Animal Health ( OIE ) standards for the quality of VS. The OIE Tool for the Evaluation of the Performance of Veterinary Services ( OIE PVS Tool ) is introduced and its relevance in assessing compliance with OIE standards to prevent the spread of pathogens through trade is highlighted .
	manualset3
97068	8	400860	13	NULL	NULL	0	NULL	OIE Tool	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , the author lists the key elements comprising good veterinary governance and discusses the World Organisation for Animal Health ( OIE ) standards for the quality of VS. The OIE Tool for the Evaluation of the Performance of Veterinary Services ( OIE PVS Tool ) is introduced and its relevance in assessing compliance with OIE standards to prevent the spread of pathogens through trade is highlighted .
	manualset3
97069	9	400860	13	NULL	NULL	0	NULL	Evaluation of the Performance of Veterinary Services ( OIE PVS Tool ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , the author lists the key elements comprising good veterinary governance and discusses the World Organisation for Animal Health ( OIE ) standards for the quality of VS. The OIE Tool for the Evaluation of the Performance of Veterinary Services ( OIE PVS Tool ) is introduced and its relevance in assessing compliance with OIE standards to prevent the spread of pathogens through trade is highlighted .
	manualset3
97070	10	400860	13	NULL	NULL	0	NULL	relevance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , the author lists the key elements comprising good veterinary governance and discusses the World Organisation for Animal Health ( OIE ) standards for the quality of VS. The OIE Tool for the Evaluation of the Performance of Veterinary Services ( OIE PVS Tool ) is introduced and its relevance in assessing compliance with OIE standards to prevent the spread of pathogens through trade is highlighted .
	manualset3
97071	11	400860	13	NULL	NULL	0	NULL	compliance with OIE standards	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , the author lists the key elements comprising good veterinary governance and discusses the World Organisation for Animal Health ( OIE ) standards for the quality of VS. The OIE Tool for the Evaluation of the Performance of Veterinary Services ( OIE PVS Tool ) is introduced and its relevance in assessing compliance with OIE standards to prevent the spread of pathogens through trade is highlighted .
	manualset3
97072	12	400860	13	NULL	NULL	0	NULL	pathogens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , the author lists the key elements comprising good veterinary governance and discusses the World Organisation for Animal Health ( OIE ) standards for the quality of VS. The OIE Tool for the Evaluation of the Performance of Veterinary Services ( OIE PVS Tool ) is introduced and its relevance in assessing compliance with OIE standards to prevent the spread of pathogens through trade is highlighted .
	manualset3
97073	13	400860	13	NULL	NULL	0	NULL	trade	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , the author lists the key elements comprising good veterinary governance and discusses the World Organisation for Animal Health ( OIE ) standards for the quality of VS. The OIE Tool for the Evaluation of the Performance of Veterinary Services ( OIE PVS Tool ) is introduced and its relevance in assessing compliance with OIE standards to prevent the spread of pathogens through trade is highlighted .
	manualset3
97074	1	400861	13	NULL	NULL	0	NULL	paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , the isotope ratios of main producers and consumers of a Mediterranean lagoon were examined in order to elucidate the fate of anthropogenic inputs from the main watercourse flowing into the lagoon .
	manualset3
97075	2	400861	13	NULL	NULL	0	NULL	isotope ratios	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , the isotope ratios of main producers and consumers of a Mediterranean lagoon were examined in order to elucidate the fate of anthropogenic inputs from the main watercourse flowing into the lagoon .
	manualset3
97076	3	400861	13	NULL	NULL	0	NULL	producers	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , the isotope ratios of main producers and consumers of a Mediterranean lagoon were examined in order to elucidate the fate of anthropogenic inputs from the main watercourse flowing into the lagoon .
	manualset3
97077	4	400861	13	NULL	NULL	0	NULL	consumers	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , the isotope ratios of main producers and consumers of a Mediterranean lagoon were examined in order to elucidate the fate of anthropogenic inputs from the main watercourse flowing into the lagoon .
	manualset3
97078	5	400861	13	NULL	NULL	NULL	NULL	Mediterranean lagoon 	GeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this paper , the isotope ratios of main producers and consumers of a Mediterranean lagoon were examined in order to elucidate the fate of anthropogenic inputs from the main watercourse flowing into the lagoon .
	manualset3
97079	6	400861	13	NULL	NULL	0	NULL	order	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , the isotope ratios of main producers and consumers of a Mediterranean lagoon were examined in order to elucidate the fate of anthropogenic inputs from the main watercourse flowing into the lagoon .
	manualset3
97080	7	400861	13	NULL	NULL	0	NULL	fate 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , the isotope ratios of main producers and consumers of a Mediterranean lagoon were examined in order to elucidate the fate of anthropogenic inputs from the main watercourse flowing into the lagoon .
	manualset3
97081	8	400861	13	NULL	NULL	0	NULL	anthropogenic inputs	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , the isotope ratios of main producers and consumers of a Mediterranean lagoon were examined in order to elucidate the fate of anthropogenic inputs from the main watercourse flowing into the lagoon .
	manualset3
97082	9	400861	13	NULL	NULL	0	NULL	watercourse 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , the isotope ratios of main producers and consumers of a Mediterranean lagoon were examined in order to elucidate the fate of anthropogenic inputs from the main watercourse flowing into the lagoon .
	manualset3
97083	10	400861	13	NULL	NULL	0	NULL	lagoon	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , the isotope ratios of main producers and consumers of a Mediterranean lagoon were examined in order to elucidate the fate of anthropogenic inputs from the main watercourse flowing into the lagoon .
	manualset3
97084	1	400862	13	NULL	NULL	0	NULL	paper 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we investigate the focalization properties of single-element transducers at low frequencies ( 300 to 1000 kHz ) through primate and human skulls .
	manualset3
97085	2	400862	13	NULL	NULL	0	NULL	focalization properties	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we investigate the focalization properties of single-element transducers at low frequencies ( 300 to 1000 kHz ) through primate and human skulls .
	manualset3
97086	3	400862	13	NULL	NULL	0	NULL	single-element transducers	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we investigate the focalization properties of single-element transducers at low frequencies ( 300 to 1000 kHz ) through primate and human skulls .
	manualset3
97087	4	400862	13	NULL	NULL	0	NULL	low frequencies ( 300 to 1000 kHz )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we investigate the focalization properties of single-element transducers at low frequencies ( 300 to 1000 kHz ) through primate and human skulls .
	manualset3
97088	5	400862	13	NULL	NULL	0	NULL	primate skulls	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we investigate the focalization properties of single-element transducers at low frequencies ( 300 to 1000 kHz ) through primate and human skulls .
	manualset3
97089	6	400862	13	NULL	NULL	0	NULL	human skulls	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we investigate the focalization properties of single-element transducers at low frequencies ( 300 to 1000 kHz ) through primate and human skulls .
	manualset3
97090	1	400863	13	NULL	NULL	0	NULL	 paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we present a patient with ulcerative colitis who developed Acremonium kiliense fungemia associated with infliximab therapy while receiving total parenteral nutrition .
	manualset3
97091	2	400863	13	NULL	NULL	0	NULL	 patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we present a patient with ulcerative colitis who developed Acremonium kiliense fungemia associated with infliximab therapy while receiving total parenteral nutrition .
	manualset3
97092	3	400863	13	NULL	NULL	0	NULL	ulcerative colitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we present a patient with ulcerative colitis who developed Acremonium kiliense fungemia associated with infliximab therapy while receiving total parenteral nutrition .
	manualset3
97093	4	400863	13	NULL	NULL	0	NULL	Acremonium kiliense fungemia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we present a patient with ulcerative colitis who developed Acremonium kiliense fungemia associated with infliximab therapy while receiving total parenteral nutrition .
	manualset3
97094	5	400863	13	NULL	NULL	0	NULL	infliximab therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we present a patient with ulcerative colitis who developed Acremonium kiliense fungemia associated with infliximab therapy while receiving total parenteral nutrition .
	manualset3
97095	6	400863	13	NULL	NULL	0	NULL	total parenteral nutrition	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we present a patient with ulcerative colitis who developed Acremonium kiliense fungemia associated with infliximab therapy while receiving total parenteral nutrition .
	manualset3
97096	1	400864	13	NULL	NULL	0	NULL	paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we propose a two-stage feature selection method , which uses information gain to implement a gene-ranking process , and combines an improved particle swarm optimization with the K-nearest neighbor method and support vector machine classifiers to calculate the classification accuracy .
	manualset3
97097	2	400864	13	NULL	NULL	0	NULL	two-stage feature selection method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we propose a two-stage feature selection method , which uses information gain to implement a gene-ranking process , and combines an improved particle swarm optimization with the K-nearest neighbor method and support vector machine classifiers to calculate the classification accuracy .
	manualset3
97098	3	400864	13	NULL	NULL	0	NULL	information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we propose a two-stage feature selection method , which uses information gain to implement a gene-ranking process , and combines an improved particle swarm optimization with the K-nearest neighbor method and support vector machine classifiers to calculate the classification accuracy .
	manualset3
97099	4	400864	13	NULL	NULL	NULL	NULL	gene-ranking process	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this paper , we propose a two-stage feature selection method , which uses information gain to implement a gene-ranking process , and combines an improved particle swarm optimization with the K-nearest neighbor method and support vector machine classifiers to calculate the classification accuracy .
	manualset3
97100	5	400864	13	NULL	NULL	NULL	NULL	particle swarm optimization	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this paper , we propose a two-stage feature selection method , which uses information gain to implement a gene-ranking process , and combines an improved particle swarm optimization with the K-nearest neighbor method and support vector machine classifiers to calculate the classification accuracy .
	manualset3
97101	6	400864	13	NULL	NULL	NULL	NULL	K-nearest neighbor method	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this paper , we propose a two-stage feature selection method , which uses information gain to implement a gene-ranking process , and combines an improved particle swarm optimization with the K-nearest neighbor method and support vector machine classifiers to calculate the classification accuracy .
	manualset3
97102	7	400864	13	NULL	NULL	0	NULL	support vector machine classifiers 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we propose a two-stage feature selection method , which uses information gain to implement a gene-ranking process , and combines an improved particle swarm optimization with the K-nearest neighbor method and support vector machine classifiers to calculate the classification accuracy .
	manualset3
97103	8	400864	13	NULL	NULL	0	NULL	classification accuracy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we propose a two-stage feature selection method , which uses information gain to implement a gene-ranking process , and combines an improved particle swarm optimization with the K-nearest neighbor method and support vector machine classifiers to calculate the classification accuracy .
	manualset3
97104	1	400865	13	NULL	NULL	0	NULL	paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we show that the proposed method , Individual Kernel TensorFaces , produces the better discrimination power for classification .
	manualset3
97105	2	400865	13	NULL	NULL	0	NULL	 method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we show that the proposed method , Individual Kernel TensorFaces , produces the better discrimination power for classification .
	manualset3
97106	3	400865	13	NULL	NULL	0	NULL	Individual Kernel TensorFaces	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we show that the proposed method , Individual Kernel TensorFaces , produces the better discrimination power for classification .
	manualset3
97107	4	400865	13	NULL	NULL	0	NULL	discrimination power	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we show that the proposed method , Individual Kernel TensorFaces , produces the better discrimination power for classification .
	manualset3
97108	5	400865	13	NULL	NULL	0	NULL	classification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we show that the proposed method , Individual Kernel TensorFaces , produces the better discrimination power for classification .
	manualset3
97129	1	400866	13	NULL	NULL	0	NULL	 paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we will demonstrate our hypothesis that the introduction of ethanol into the water nanofilm alters the properties of the interfacial water , resulting in changes of the peptide nanostructures self-assembled on the substrate .
	manualset3
97130	2	400866	13	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we will demonstrate our hypothesis that the introduction of ethanol into the water nanofilm alters the properties of the interfacial water , resulting in changes of the peptide nanostructures self-assembled on the substrate .
	manualset3
97131	3	400866	13	NULL	NULL	0	NULL	 introduction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we will demonstrate our hypothesis that the introduction of ethanol into the water nanofilm alters the properties of the interfacial water , resulting in changes of the peptide nanostructures self-assembled on the substrate .
	manualset3
97132	4	400866	13	NULL	NULL	0	NULL	ethanol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we will demonstrate our hypothesis that the introduction of ethanol into the water nanofilm alters the properties of the interfacial water , resulting in changes of the peptide nanostructures self-assembled on the substrate .
	manualset3
97133	5	400866	13	NULL	NULL	0	NULL	water nanofilm	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we will demonstrate our hypothesis that the introduction of ethanol into the water nanofilm alters the properties of the interfacial water , resulting in changes of the peptide nanostructures self-assembled on the substrate .
	manualset3
97140	6	400866	13	NULL	NULL	0	NULL	interfacial water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we will demonstrate our hypothesis that the introduction of ethanol into the water nanofilm alters the properties of the interfacial water , resulting in changes of the peptide nanostructures self-assembled on the substrate .
	manualset3
97141	7	400866	13	NULL	NULL	0	NULL	changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we will demonstrate our hypothesis that the introduction of ethanol into the water nanofilm alters the properties of the interfacial water , resulting in changes of the peptide nanostructures self-assembled on the substrate .
	manualset3
97144	8	400866	13	NULL	NULL	0	NULL	peptide nanostructures 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we will demonstrate our hypothesis that the introduction of ethanol into the water nanofilm alters the properties of the interfacial water , resulting in changes of the peptide nanostructures self-assembled on the substrate .
	manualset3
97195	9	400866	13	NULL	NULL	0	NULL	 substrate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper , we will demonstrate our hypothesis that the introduction of ethanol into the water nanofilm alters the properties of the interfacial water , resulting in changes of the peptide nanostructures self-assembled on the substrate .
	manualset3
97197	1	400867	13	NULL	NULL	0	NULL	paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper I will discuss some of the more common pitfalls inherent in attempts to introduce clinical supervision to hospital wards or community teams .
	manualset3
97199	2	400867	13	NULL	NULL	0	NULL	pitfalls	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper I will discuss some of the more common pitfalls inherent in attempts to introduce clinical supervision to hospital wards or community teams .
	manualset3
97202	3	400867	13	NULL	NULL	NULL	NULL	attempts	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this paper I will discuss some of the more common pitfalls inherent in attempts to introduce clinical supervision to hospital wards or community teams .
	manualset3
97204	4	400867	13	NULL	NULL	0	NULL	clinical supervision	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper I will discuss some of the more common pitfalls inherent in attempts to introduce clinical supervision to hospital wards or community teams .
	manualset3
97206	5	400867	13	NULL	NULL	0	NULL	 hospital wards	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper I will discuss some of the more common pitfalls inherent in attempts to introduce clinical supervision to hospital wards or community teams .
	manualset3
97208	6	400867	13	NULL	NULL	0	NULL	community teams	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper I will discuss some of the more common pitfalls inherent in attempts to introduce clinical supervision to hospital wards or community teams .
	manualset3
97338	1	400868	13	NULL	NULL	0	NULL	paper 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we describe the isolation , sequencing , and analysis of 15 omitted559 bp of chromosomal DNA , containing the potential nonactin biosynthesis gene cluster , from S. griseus subsp .
	manualset3
97339	2	400868	13	NULL	NULL	0	NULL	isolation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we describe the isolation , sequencing , and analysis of 15 omitted559 bp of chromosomal DNA , containing the potential nonactin biosynthesis gene cluster , from S. griseus subsp .
	manualset3
97340	3	400868	13	NULL	NULL	0	NULL	sequencing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we describe the isolation , sequencing , and analysis of 15 omitted559 bp of chromosomal DNA , containing the potential nonactin biosynthesis gene cluster , from S. griseus subsp .
	manualset3
97341	4	400868	13	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we describe the isolation , sequencing , and analysis of 15 omitted559 bp of chromosomal DNA , containing the potential nonactin biosynthesis gene cluster , from S. griseus subsp .
	manualset3
97342	5	400868	13	NULL	NULL	0	NULL	15 omitted559 bp of chromosomal DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we describe the isolation , sequencing , and analysis of 15 omitted559 bp of chromosomal DNA , containing the potential nonactin biosynthesis gene cluster , from S. griseus subsp .
	manualset3
97343	6	400868	13	NULL	NULL	0	NULL	nonactin biosynthesis gene cluster	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we describe the isolation , sequencing , and analysis of 15 omitted559 bp of chromosomal DNA , containing the potential nonactin biosynthesis gene cluster , from S. griseus subsp .
	manualset3
97344	7	400868	13	NULL	NULL	0	NULL	S. griseus subsp	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we describe the isolation , sequencing , and analysis of 15 omitted559 bp of chromosomal DNA , containing the potential nonactin biosynthesis gene cluster , from S. griseus subsp .
	manualset3
97345	1	400869	13	NULL	NULL	0	NULL	 paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we present the updated ( March 1996 ) compilation of eukaryotic 5D rRNA and 5S rDNA sequences .
	manualset3
97346	2	400869	13	NULL	NULL	0	NULL	March 1996 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we present the updated ( March 1996 ) compilation of eukaryotic 5D rRNA and 5S rDNA sequences .
	manualset3
97347	3	400869	13	NULL	NULL	0	NULL	compilation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we present the updated ( March 1996 ) compilation of eukaryotic 5D rRNA and 5S rDNA sequences .
	manualset3
97348	4	400869	13	NULL	NULL	0	NULL	eukaryotic 5D rRNA sequences 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we present the updated ( March 1996 ) compilation of eukaryotic 5D rRNA and 5S rDNA sequences .
	manualset3
97349	5	400869	13	NULL	NULL	0	NULL	eukaryotic 5S rDNA sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we present the updated ( March 1996 ) compilation of eukaryotic 5D rRNA and 5S rDNA sequences .
	manualset3
97350	1	400870	13	NULL	NULL	0	NULL	paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we report concentrations of lead , cadmium , mercury , and selenium in breast feathers of common terns ( Sterna hirundo ) and roseate terns ( S. dougallii ) trapped during incubation at breeding colonies in New York and Massachusetts .
	manualset3
97351	2	400870	13	NULL	NULL	0	NULL	 concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we report concentrations of lead , cadmium , mercury , and selenium in breast feathers of common terns ( Sterna hirundo ) and roseate terns ( S. dougallii ) trapped during incubation at breeding colonies in New York and Massachusetts .
	manualset3
97352	3	400870	13	NULL	NULL	0	NULL	lead	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we report concentrations of lead , cadmium , mercury , and selenium in breast feathers of common terns ( Sterna hirundo ) and roseate terns ( S. dougallii ) trapped during incubation at breeding colonies in New York and Massachusetts .
	manualset3
97353	4	400870	13	NULL	NULL	0	NULL	cadmium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we report concentrations of lead , cadmium , mercury , and selenium in breast feathers of common terns ( Sterna hirundo ) and roseate terns ( S. dougallii ) trapped during incubation at breeding colonies in New York and Massachusetts .
	manualset3
97354	5	400870	13	NULL	NULL	0	NULL	 mercury	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we report concentrations of lead , cadmium , mercury , and selenium in breast feathers of common terns ( Sterna hirundo ) and roseate terns ( S. dougallii ) trapped during incubation at breeding colonies in New York and Massachusetts .
	manualset3
97355	6	400870	13	NULL	NULL	0	NULL	selenium 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we report concentrations of lead , cadmium , mercury , and selenium in breast feathers of common terns ( Sterna hirundo ) and roseate terns ( S. dougallii ) trapped during incubation at breeding colonies in New York and Massachusetts .
	manualset3
97356	7	400870	13	NULL	NULL	0	NULL	breast feathers 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we report concentrations of lead , cadmium , mercury , and selenium in breast feathers of common terns ( Sterna hirundo ) and roseate terns ( S. dougallii ) trapped during incubation at breeding colonies in New York and Massachusetts .
	manualset3
97357	8	400870	13	NULL	NULL	0	NULL	common terns	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we report concentrations of lead , cadmium , mercury , and selenium in breast feathers of common terns ( Sterna hirundo ) and roseate terns ( S. dougallii ) trapped during incubation at breeding colonies in New York and Massachusetts .
	manualset3
97358	9	400870	13	NULL	NULL	0	NULL	Sterna hirundo	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we report concentrations of lead , cadmium , mercury , and selenium in breast feathers of common terns ( Sterna hirundo ) and roseate terns ( S. dougallii ) trapped during incubation at breeding colonies in New York and Massachusetts .
	manualset3
97359	10	400870	13	NULL	NULL	0	NULL	roseate terns	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we report concentrations of lead , cadmium , mercury , and selenium in breast feathers of common terns ( Sterna hirundo ) and roseate terns ( S. dougallii ) trapped during incubation at breeding colonies in New York and Massachusetts .
	manualset3
97360	11	400870	13	NULL	NULL	0	NULL	incubation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we report concentrations of lead , cadmium , mercury , and selenium in breast feathers of common terns ( Sterna hirundo ) and roseate terns ( S. dougallii ) trapped during incubation at breeding colonies in New York and Massachusetts .
	manualset3
97361	12	400870	13	NULL	NULL	0	NULL	breeding colonies	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we report concentrations of lead , cadmium , mercury , and selenium in breast feathers of common terns ( Sterna hirundo ) and roseate terns ( S. dougallii ) trapped during incubation at breeding colonies in New York and Massachusetts .
	manualset3
97362	13	400870	13	NULL	NULL	0	NULL	 New York	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we report concentrations of lead , cadmium , mercury , and selenium in breast feathers of common terns ( Sterna hirundo ) and roseate terns ( S. dougallii ) trapped during incubation at breeding colonies in New York and Massachusetts .
	manualset3
97363	14	400870	13	NULL	NULL	0	NULL	Massachusetts	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we report concentrations of lead , cadmium , mercury , and selenium in breast feathers of common terns ( Sterna hirundo ) and roseate terns ( S. dougallii ) trapped during incubation at breeding colonies in New York and Massachusetts .
	manualset3
97364	1	400871	13	NULL	NULL	0	NULL	paper 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we report on studies of platelet adhesion to several fibrinogen gamma chain variants under physiological flow conditions .
	manualset3
97365	2	400871	13	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we report on studies of platelet adhesion to several fibrinogen gamma chain variants under physiological flow conditions .
	manualset3
97366	3	400871	13	NULL	NULL	0	NULL	platelet adhesion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we report on studies of platelet adhesion to several fibrinogen gamma chain variants under physiological flow conditions .
	manualset3
97367	4	400871	13	NULL	NULL	0	NULL	fibrinogen gamma chain variants	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we report on studies of platelet adhesion to several fibrinogen gamma chain variants under physiological flow conditions .
	manualset3
97368	5	400871	13	NULL	NULL	0	NULL	physiological flow conditions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we report on studies of platelet adhesion to several fibrinogen gamma chain variants under physiological flow conditions .
	manualset3
97369	1	400872	13	NULL	NULL	0	NULL	paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we report that collagen IV is a strong candidate for the factor IX binding site on endothelial cells .
	manualset3
97370	2	400872	13	NULL	NULL	0	NULL	collagen IV	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we report that collagen IV is a strong candidate for the factor IX binding site on endothelial cells .
	manualset3
97371	3	400872	13	NULL	NULL	0	NULL	candidate	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we report that collagen IV is a strong candidate for the factor IX binding site on endothelial cells .
	manualset3
97372	4	400872	13	NULL	NULL	0	NULL	factor IX binding site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we report that collagen IV is a strong candidate for the factor IX binding site on endothelial cells .
	manualset3
97373	5	400872	13	NULL	NULL	0	NULL	endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we report that collagen IV is a strong candidate for the factor IX binding site on endothelial cells .
	manualset3
97374	1	400873	13	NULL	NULL	0	NULL	paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we review the evidence for the notion that a context memory deficit makes an important contribution to the amnesia in these patients .
	manualset3
97375	2	400873	13	NULL	NULL	0	NULL	review 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we review the evidence for the notion that a context memory deficit makes an important contribution to the amnesia in these patients .
	manualset3
97376	3	400873	13	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we review the evidence for the notion that a context memory deficit makes an important contribution to the amnesia in these patients .
	manualset3
97377	4	400873	13	NULL	NULL	0	NULL	notion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we review the evidence for the notion that a context memory deficit makes an important contribution to the amnesia in these patients .
	manualset3
97378	5	400873	13	NULL	NULL	0	NULL	context memory deficit 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we review the evidence for the notion that a context memory deficit makes an important contribution to the amnesia in these patients .
	manualset3
97379	6	400873	13	NULL	NULL	0	NULL	contribution 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we review the evidence for the notion that a context memory deficit makes an important contribution to the amnesia in these patients .
	manualset3
97380	7	400873	13	NULL	NULL	0	NULL	amnesia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we review the evidence for the notion that a context memory deficit makes an important contribution to the amnesia in these patients .
	manualset3
97381	8	400873	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we review the evidence for the notion that a context memory deficit makes an important contribution to the amnesia in these patients .
	manualset3
97382	1	400874	13	NULL	NULL	0	NULL	paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we shall derive an estimate for that variation with a similar model as used for the shot noise effect in the lithography step .
	manualset3
97383	2	400874	13	NULL	NULL	0	NULL	 estimate	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we shall derive an estimate for that variation with a similar model as used for the shot noise effect in the lithography step .
	manualset3
97384	3	400874	13	NULL	NULL	0	NULL	variation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we shall derive an estimate for that variation with a similar model as used for the shot noise effect in the lithography step .
	manualset3
97385	4	400874	13	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we shall derive an estimate for that variation with a similar model as used for the shot noise effect in the lithography step .
	manualset3
97386	5	400874	13	NULL	NULL	0	NULL	 shot noise effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we shall derive an estimate for that variation with a similar model as used for the shot noise effect in the lithography step .
	manualset3
97387	6	400874	13	NULL	NULL	0	NULL	 lithography step	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we shall derive an estimate for that variation with a similar model as used for the shot noise effect in the lithography step .
	manualset3
97388	1	400875	13	NULL	NULL	0	NULL	part 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this part , we show that the complex pattern described there might be explained by an analytic model , in terms of a simple dynamical system , with few assumptions concerning motivation and learning .
	manualset3
97389	2	400875	13	NULL	NULL	0	NULL	complex pattern	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this part , we show that the complex pattern described there might be explained by an analytic model , in terms of a simple dynamical system , with few assumptions concerning motivation and learning .
	manualset3
97390	3	400875	13	NULL	NULL	0	NULL	analytic model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this part , we show that the complex pattern described there might be explained by an analytic model , in terms of a simple dynamical system , with few assumptions concerning motivation and learning .
	manualset3
97391	4	400875	13	NULL	NULL	0	NULL	dynamical system	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this part , we show that the complex pattern described there might be explained by an analytic model , in terms of a simple dynamical system , with few assumptions concerning motivation and learning .
	manualset3
97392	5	400875	13	NULL	NULL	0	NULL	assumptions	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this part , we show that the complex pattern described there might be explained by an analytic model , in terms of a simple dynamical system , with few assumptions concerning motivation and learning .
	manualset3
97393	6	400875	13	NULL	NULL	0	NULL	motivation 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this part , we show that the complex pattern described there might be explained by an analytic model , in terms of a simple dynamical system , with few assumptions concerning motivation and learning .
	manualset3
97394	7	400875	13	NULL	NULL	0	NULL	learning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this part , we show that the complex pattern described there might be explained by an analytic model , in terms of a simple dynamical system , with few assumptions concerning motivation and learning .
	manualset3
97395	1	400876	13	NULL	NULL	0	NULL	population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this population , approximately one third of children newly diagnosed with epilepsy experienced treatment failure with the first antiepileptic drug used .
	manualset3
97396	2	400876	13	NULL	NULL	0	NULL	one third	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this population , approximately one third of children newly diagnosed with epilepsy experienced treatment failure with the first antiepileptic drug used .
	manualset3
97397	3	400876	13	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this population , approximately one third of children newly diagnosed with epilepsy experienced treatment failure with the first antiepileptic drug used .
	manualset3
97398	4	400876	13	NULL	NULL	0	NULL	epilepsy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In this population , approximately one third of children newly diagnosed with epilepsy experienced treatment failure with the first antiepileptic drug used .
	manualset3
97399	5	400876	13	NULL	NULL	0	NULL	treatment failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this population , approximately one third of children newly diagnosed with epilepsy experienced treatment failure with the first antiepileptic drug used .
	manualset3
97400	6	400876	13	NULL	NULL	0	NULL	antiepileptic drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In this population , approximately one third of children newly diagnosed with epilepsy experienced treatment failure with the first antiepileptic drug used .
	manualset3
97401	1	400877	13	NULL	NULL	0	NULL	 population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this population , we found that the risk ratio for an animal to be simultaneously affected by HD and ED is 1.67 .
	manualset3
97402	2	400877	13	NULL	NULL	0	NULL	risk ratio	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this population , we found that the risk ratio for an animal to be simultaneously affected by HD and ED is 1.67 .
	manualset3
97403	3	400877	13	NULL	NULL	NULL	NULL	animal	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this population , we found that the risk ratio for an animal to be simultaneously affected by HD and ED is 1.67 .
	manualset3
97404	4	400877	13	NULL	NULL	NULL	NULL	HD	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this population , we found that the risk ratio for an animal to be simultaneously affected by HD and ED is 1.67 .
	manualset3
97405	5	400877	13	NULL	NULL	NULL	NULL	 ED	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this population , we found that the risk ratio for an animal to be simultaneously affected by HD and ED is 1.67 .
	manualset3
97410	6	400877	13	NULL	NULL	0	NULL	1.67	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this population , we found that the risk ratio for an animal to be simultaneously affected by HD and ED is 1.67 .
	manualset3
97411	1	400878	13	NULL	NULL	0	NULL	16S rDNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	16S rDNA was not found in the equine filarial nematode Setaria equina , using either polymerase chain reaction ( PCR ) or DNA hybridization .
	manualset3
97412	2	400878	13	NULL	NULL	0	NULL	equine filarial nematode Setaria equina	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	16S rDNA was not found in the equine filarial nematode Setaria equina , using either polymerase chain reaction ( PCR ) or DNA hybridization .
	manualset3
97413	3	400878	13	NULL	NULL	0	NULL	polymerase chain reaction ( PCR ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	16S rDNA was not found in the equine filarial nematode Setaria equina , using either polymerase chain reaction ( PCR ) or DNA hybridization .
	manualset3
97414	4	400878	13	NULL	NULL	0	NULL	DNA hybridization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	16S rDNA was not found in the equine filarial nematode Setaria equina , using either polymerase chain reaction ( PCR ) or DNA hybridization .
	manualset3
97415	1	400879	13	NULL	NULL	0	NULL	 multicenter cohort study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this prospective multicenter cohort study of early PJI managed by DAIR , factors associated with failure of the DAIR were analyzed .
	manualset3
97416	2	400879	13	NULL	NULL	0	NULL	PJI	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this prospective multicenter cohort study of early PJI managed by DAIR , factors associated with failure of the DAIR were analyzed .
	manualset3
97417	3	400879	13	NULL	NULL	0	NULL	DAIR	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this prospective multicenter cohort study of early PJI managed by DAIR , factors associated with failure of the DAIR were analyzed .
	manualset3
97418	4	400879	13	NULL	NULL	0	NULL	factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this prospective multicenter cohort study of early PJI managed by DAIR , factors associated with failure of the DAIR were analyzed .
	manualset3
97419	5	400879	13	NULL	NULL	NULL	NULL	failure	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this prospective multicenter cohort study of early PJI managed by DAIR , factors associated with failure of the DAIR were analyzed .
	manualset3
97420	6	400879	13	NULL	NULL	0	NULL	DAIR 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this prospective multicenter cohort study of early PJI managed by DAIR , factors associated with failure of the DAIR were analyzed .
	manualset3
97421	1	400880	13	NULL	NULL	0	NULL	provirus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this provirus the v-myc sequences are located at the 3 ' end of the pol gene , replacing pol and env sequences .
	manualset3
97422	2	400880	13	NULL	NULL	0	NULL	v-myc sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this provirus the v-myc sequences are located at the 3 ' end of the pol gene , replacing pol and env sequences .
	manualset3
97423	3	400880	13	NULL	NULL	0	NULL	3 ' end of the pol gene	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this provirus the v-myc sequences are located at the 3 ' end of the pol gene , replacing pol and env sequences .
	manualset3
97424	4	400880	13	NULL	NULL	0	NULL	pol sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this provirus the v-myc sequences are located at the 3 ' end of the pol gene , replacing pol and env sequences .
	manualset3
97425	5	400880	13	NULL	NULL	0	NULL	env sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this provirus the v-myc sequences are located at the 3 ' end of the pol gene , replacing pol and env sequences .
	manualset3
97426	1	400881	13	NULL	NULL	0	NULL	open-label , three-way crossover study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this randomized , open-label , three-way crossover study , 24 healthy men received three single-dose oral treatments : 2 mg everolimus , 20 mg atorvastatin ( n = 12 ) or 20 mg pravastatin ( n = 12 ) , and the respective statin coadministered with everolimus .
	manualset3
97427	2	400881	13	NULL	NULL	0	NULL	24 healthy men 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this randomized , open-label , three-way crossover study , 24 healthy men received three single-dose oral treatments : 2 mg everolimus , 20 mg atorvastatin ( n = 12 ) or 20 mg pravastatin ( n = 12 ) , and the respective statin coadministered with everolimus .
	manualset3
97428	3	400881	13	NULL	NULL	0	NULL	three single-dose oral treatments 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this randomized , open-label , three-way crossover study , 24 healthy men received three single-dose oral treatments : 2 mg everolimus , 20 mg atorvastatin ( n = 12 ) or 20 mg pravastatin ( n = 12 ) , and the respective statin coadministered with everolimus .
	manualset3
97429	4	400881	13	NULL	NULL	0	NULL	2 mg everolimus 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In this randomized , open-label , three-way crossover study , 24 healthy men received three single-dose oral treatments : 2 mg everolimus , 20 mg atorvastatin ( n = 12 ) or 20 mg pravastatin ( n = 12 ) , and the respective statin coadministered with everolimus .
	manualset3
97430	5	400881	13	NULL	NULL	0	NULL	20 mg atorvastatin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In this randomized , open-label , three-way crossover study , 24 healthy men received three single-dose oral treatments : 2 mg everolimus , 20 mg atorvastatin ( n = 12 ) or 20 mg pravastatin ( n = 12 ) , and the respective statin coadministered with everolimus .
	manualset3
97431	6	400881	13	NULL	NULL	NULL	NULL	n = 12 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this randomized , open-label , three-way crossover study , 24 healthy men received three single-dose oral treatments : 2 mg everolimus , 20 mg atorvastatin ( n = 12 ) or 20 mg pravastatin ( n = 12 ) , and the respective statin coadministered with everolimus .
	manualset3
97432	7	400881	13	NULL	NULL	0	NULL	20 mg pravastatin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In this randomized , open-label , three-way crossover study , 24 healthy men received three single-dose oral treatments : 2 mg everolimus , 20 mg atorvastatin ( n = 12 ) or 20 mg pravastatin ( n = 12 ) , and the respective statin coadministered with everolimus .
	manualset3
97433	8	400881	13	NULL	NULL	0	NULL	n = 12	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this randomized , open-label , three-way crossover study , 24 healthy men received three single-dose oral treatments : 2 mg everolimus , 20 mg atorvastatin ( n = 12 ) or 20 mg pravastatin ( n = 12 ) , and the respective statin coadministered with everolimus .
	manualset3
97434	9	400881	13	NULL	NULL	NULL	NULL	statin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this randomized , open-label , three-way crossover study , 24 healthy men received three single-dose oral treatments : 2 mg everolimus , 20 mg atorvastatin ( n = 12 ) or 20 mg pravastatin ( n = 12 ) , and the respective statin coadministered with everolimus .
	manualset3
97435	10	400881	13	NULL	NULL	0	NULL	everolimus	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In this randomized , open-label , three-way crossover study , 24 healthy men received three single-dose oral treatments : 2 mg everolimus , 20 mg atorvastatin ( n = 12 ) or 20 mg pravastatin ( n = 12 ) , and the respective statin coadministered with everolimus .
	manualset3
97436	1	400882	13	NULL	NULL	0	NULL	photophysical investigations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this regards , the photophysical investigations by means of fluorescence , flash photolysis , and transient-absorption spectroscopy have manifested a clear dependence between charge transfer kinetics and spatial arrangement .
	manualset3
97437	2	400882	13	NULL	NULL	0	NULL	means	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this regards , the photophysical investigations by means of fluorescence , flash photolysis , and transient-absorption spectroscopy have manifested a clear dependence between charge transfer kinetics and spatial arrangement .
	manualset3
97438	3	400882	13	NULL	NULL	0	NULL	fluorescence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this regards , the photophysical investigations by means of fluorescence , flash photolysis , and transient-absorption spectroscopy have manifested a clear dependence between charge transfer kinetics and spatial arrangement .
	manualset3
97439	4	400882	13	NULL	NULL	0	NULL	 flash photolysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this regards , the photophysical investigations by means of fluorescence , flash photolysis , and transient-absorption spectroscopy have manifested a clear dependence between charge transfer kinetics and spatial arrangement .
	manualset3
97440	5	400882	13	NULL	NULL	0	NULL	 transient-absorption spectroscopy 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this regards , the photophysical investigations by means of fluorescence , flash photolysis , and transient-absorption spectroscopy have manifested a clear dependence between charge transfer kinetics and spatial arrangement .
	manualset3
97441	6	400882	13	NULL	NULL	0	NULL	 dependence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this regards , the photophysical investigations by means of fluorescence , flash photolysis , and transient-absorption spectroscopy have manifested a clear dependence between charge transfer kinetics and spatial arrangement .
	manualset3
97442	7	400882	13	NULL	NULL	NULL	NULL	charge transfer kinetics	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this regards , the photophysical investigations by means of fluorescence , flash photolysis , and transient-absorption spectroscopy have manifested a clear dependence between charge transfer kinetics and spatial arrangement .
	manualset3
97443	8	400882	13	NULL	NULL	0	NULL	 spatial arrangement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this regards , the photophysical investigations by means of fluorescence , flash photolysis , and transient-absorption spectroscopy have manifested a clear dependence between charge transfer kinetics and spatial arrangement .
	manualset3
97444	1	400883	13	NULL	NULL	0	NULL	 report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report , a representative PE_PGRS gene ( Rv1818c/PE _ PGRS33 ) was selected to investigate the role of these proteins .
	manualset3
97445	2	400883	13	NULL	NULL	NULL	NULL	PE_PGRS gene ( Rv1818c/PE _ PGRS33 ) 	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this report , a representative PE_PGRS gene ( Rv1818c/PE _ PGRS33 ) was selected to investigate the role of these proteins .
	manualset3
97446	3	400883	13	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report , a representative PE_PGRS gene ( Rv1818c/PE _ PGRS33 ) was selected to investigate the role of these proteins .
	manualset3
97447	4	400883	13	NULL	NULL	0	NULL	proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report , a representative PE_PGRS gene ( Rv1818c/PE _ PGRS33 ) was selected to investigate the role of these proteins .
	manualset3
97448	1	400884	13	NULL	NULL	0	NULL	report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report , conditions for the isolation of rat liver plasma membranes containing PDE that is sensitive to in vitro insulin stimulation and the involvement of CaM in insulin stimulation of PDE were investigated .
	manualset3
97449	2	400884	13	NULL	NULL	0	NULL	conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report , conditions for the isolation of rat liver plasma membranes containing PDE that is sensitive to in vitro insulin stimulation and the involvement of CaM in insulin stimulation of PDE were investigated .
	manualset3
97450	3	400884	13	NULL	NULL	0	NULL	isolation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report , conditions for the isolation of rat liver plasma membranes containing PDE that is sensitive to in vitro insulin stimulation and the involvement of CaM in insulin stimulation of PDE were investigated .
	manualset3
97451	4	400884	13	NULL	NULL	0	NULL	rat liver plasma membranes 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report , conditions for the isolation of rat liver plasma membranes containing PDE that is sensitive to in vitro insulin stimulation and the involvement of CaM in insulin stimulation of PDE were investigated .
	manualset3
97452	5	400884	13	NULL	NULL	0	NULL	PDE	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report , conditions for the isolation of rat liver plasma membranes containing PDE that is sensitive to in vitro insulin stimulation and the involvement of CaM in insulin stimulation of PDE were investigated .
	manualset3
97453	6	400884	13	NULL	NULL	0	NULL	 in vitro insulin stimulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report , conditions for the isolation of rat liver plasma membranes containing PDE that is sensitive to in vitro insulin stimulation and the involvement of CaM in insulin stimulation of PDE were investigated .
	manualset3
97454	7	400884	13	NULL	NULL	0	NULL	involvement	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report , conditions for the isolation of rat liver plasma membranes containing PDE that is sensitive to in vitro insulin stimulation and the involvement of CaM in insulin stimulation of PDE were investigated .
	manualset3
97455	8	400884	13	NULL	NULL	0	NULL	CaM 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report , conditions for the isolation of rat liver plasma membranes containing PDE that is sensitive to in vitro insulin stimulation and the involvement of CaM in insulin stimulation of PDE were investigated .
	manualset3
97456	9	400884	13	NULL	NULL	0	NULL	insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report , conditions for the isolation of rat liver plasma membranes containing PDE that is sensitive to in vitro insulin stimulation and the involvement of CaM in insulin stimulation of PDE were investigated .
	manualset3
97457	10	400884	13	NULL	NULL	0	NULL	stimulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report , conditions for the isolation of rat liver plasma membranes containing PDE that is sensitive to in vitro insulin stimulation and the involvement of CaM in insulin stimulation of PDE were investigated .
	manualset3
97458	11	400884	13	NULL	NULL	0	NULL	PDE	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report , conditions for the isolation of rat liver plasma membranes containing PDE that is sensitive to in vitro insulin stimulation and the involvement of CaM in insulin stimulation of PDE were investigated .
	manualset3
97459	1	400885	13	NULL	NULL	0	NULL	report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report , the case of a 48-year-old woman who developed an esophageal stricture , and subsequently Barrett 's esophagus , secondary to increased intra-abdominal pressure following abdominoplasty is presented .
	manualset3
97460	2	400885	13	NULL	NULL	0	NULL	case	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report , the case of a 48-year-old woman who developed an esophageal stricture , and subsequently Barrett 's esophagus , secondary to increased intra-abdominal pressure following abdominoplasty is presented .
	manualset3
97461	3	400885	13	NULL	NULL	0	NULL	48-year-old woman	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report , the case of a 48-year-old woman who developed an esophageal stricture , and subsequently Barrett 's esophagus , secondary to increased intra-abdominal pressure following abdominoplasty is presented .
	manualset3
97462	4	400885	13	NULL	NULL	0	NULL	esophageal stricture	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report , the case of a 48-year-old woman who developed an esophageal stricture , and subsequently Barrett 's esophagus , secondary to increased intra-abdominal pressure following abdominoplasty is presented .
	manualset3
97463	5	400885	13	NULL	NULL	0	NULL	Barrett 's esophagus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report , the case of a 48-year-old woman who developed an esophageal stricture , and subsequently Barrett 's esophagus , secondary to increased intra-abdominal pressure following abdominoplasty is presented .
	manualset3
97464	6	400885	13	NULL	NULL	0	NULL	 intra-abdominal pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report , the case of a 48-year-old woman who developed an esophageal stricture , and subsequently Barrett 's esophagus , secondary to increased intra-abdominal pressure following abdominoplasty is presented .
	manualset3
97465	7	400885	13	NULL	NULL	0	NULL	abdominoplasty	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report , the case of a 48-year-old woman who developed an esophageal stricture , and subsequently Barrett 's esophagus , secondary to increased intra-abdominal pressure following abdominoplasty is presented .
	manualset3
97466	1	400886	13	NULL	NULL	0	NULL	report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report the authors describe young woman with acute stem cell leukemia which was terminal deoxyribonucleotidyl transferase positive , and involved the bone marrow and peripheral blood .
	manualset3
97467	2	400886	13	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report the authors describe young woman with acute stem cell leukemia which was terminal deoxyribonucleotidyl transferase positive , and involved the bone marrow and peripheral blood .
	manualset3
97468	3	400886	13	NULL	NULL	0	NULL	young woman	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report the authors describe young woman with acute stem cell leukemia which was terminal deoxyribonucleotidyl transferase positive , and involved the bone marrow and peripheral blood .
	manualset3
97469	4	400886	13	NULL	NULL	0	NULL	acute stem cell leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report the authors describe young woman with acute stem cell leukemia which was terminal deoxyribonucleotidyl transferase positive , and involved the bone marrow and peripheral blood .
	manualset3
97470	5	400886	13	NULL	NULL	0	NULL	deoxyribonucleotidyl transferase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report the authors describe young woman with acute stem cell leukemia which was terminal deoxyribonucleotidyl transferase positive , and involved the bone marrow and peripheral blood .
	manualset3
97471	6	400886	13	NULL	NULL	0	NULL	bone marrow 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report the authors describe young woman with acute stem cell leukemia which was terminal deoxyribonucleotidyl transferase positive , and involved the bone marrow and peripheral blood .
	manualset3
97472	7	400886	13	NULL	NULL	0	NULL	peripheral blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report the authors describe young woman with acute stem cell leukemia which was terminal deoxyribonucleotidyl transferase positive , and involved the bone marrow and peripheral blood .
	manualset3
97473	1	400887	13	NULL	NULL	0	NULL	report 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report we present evidence that the cytoplasmic ground substance , which surrounds and contains the membrane-bound compartments , may also be compartmentalized by local differentiations of its submicroscopic structure that sort subcellular particles on the basis of size .
	manualset3
97474	2	400887	13	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report we present evidence that the cytoplasmic ground substance , which surrounds and contains the membrane-bound compartments , may also be compartmentalized by local differentiations of its submicroscopic structure that sort subcellular particles on the basis of size .
	manualset3
97475	3	400887	13	NULL	NULL	0	NULL	cytoplasmic ground substance	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report we present evidence that the cytoplasmic ground substance , which surrounds and contains the membrane-bound compartments , may also be compartmentalized by local differentiations of its submicroscopic structure that sort subcellular particles on the basis of size .
	manualset3
97476	4	400887	13	NULL	NULL	0	NULL	membrane-bound compartments	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report we present evidence that the cytoplasmic ground substance , which surrounds and contains the membrane-bound compartments , may also be compartmentalized by local differentiations of its submicroscopic structure that sort subcellular particles on the basis of size .
	manualset3
97477	5	400887	13	NULL	NULL	0	NULL	differentiations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report we present evidence that the cytoplasmic ground substance , which surrounds and contains the membrane-bound compartments , may also be compartmentalized by local differentiations of its submicroscopic structure that sort subcellular particles on the basis of size .
	manualset3
97478	6	400887	13	NULL	NULL	0	NULL	submicroscopic structure	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report we present evidence that the cytoplasmic ground substance , which surrounds and contains the membrane-bound compartments , may also be compartmentalized by local differentiations of its submicroscopic structure that sort subcellular particles on the basis of size .
	manualset3
97480	8	400887	13	NULL	NULL	0	NULL	subcellular particles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report we present evidence that the cytoplasmic ground substance , which surrounds and contains the membrane-bound compartments , may also be compartmentalized by local differentiations of its submicroscopic structure that sort subcellular particles on the basis of size .
	manualset3
97481	9	400887	13	NULL	NULL	0	NULL	 size	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report we present evidence that the cytoplasmic ground substance , which surrounds and contains the membrane-bound compartments , may also be compartmentalized by local differentiations of its submicroscopic structure that sort subcellular particles on the basis of size .
	manualset3
97482	1	400888	13	NULL	NULL	0	NULL	16S rRNA gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	16S rRNA gene sequence analysis of strain TG-S248 ( T ) with sequences from Leifsonia shinshuensis DB 102 ( T ) , L. poae VKM Ac-1401 ( T ) , L. naganoensis DB 103 ( T ) , L. aquatica DSM 20146 ( T ) and L. xyli subsp .
	manualset3
97483	2	400888	13	NULL	NULL	0	NULL	sequence analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	16S rRNA gene sequence analysis of strain TG-S248 ( T ) with sequences from Leifsonia shinshuensis DB 102 ( T ) , L. poae VKM Ac-1401 ( T ) , L. naganoensis DB 103 ( T ) , L. aquatica DSM 20146 ( T ) and L. xyli subsp .
	manualset3
97484	3	400888	13	NULL	NULL	0	NULL	strain TG-S248 ( T )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	16S rRNA gene sequence analysis of strain TG-S248 ( T ) with sequences from Leifsonia shinshuensis DB 102 ( T ) , L. poae VKM Ac-1401 ( T ) , L. naganoensis DB 103 ( T ) , L. aquatica DSM 20146 ( T ) and L. xyli subsp .
	manualset3
97485	4	400888	13	NULL	NULL	0	NULL	sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	16S rRNA gene sequence analysis of strain TG-S248 ( T ) with sequences from Leifsonia shinshuensis DB 102 ( T ) , L. poae VKM Ac-1401 ( T ) , L. naganoensis DB 103 ( T ) , L. aquatica DSM 20146 ( T ) and L. xyli subsp .
	manualset3
97486	5	400888	13	NULL	NULL	0	NULL	Leifsonia shinshuensis DB 102 ( T )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	16S rRNA gene sequence analysis of strain TG-S248 ( T ) with sequences from Leifsonia shinshuensis DB 102 ( T ) , L. poae VKM Ac-1401 ( T ) , L. naganoensis DB 103 ( T ) , L. aquatica DSM 20146 ( T ) and L. xyli subsp .
	manualset3
97487	6	400888	13	NULL	NULL	0	NULL	L. poae VKM Ac-1401 ( T )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	16S rRNA gene sequence analysis of strain TG-S248 ( T ) with sequences from Leifsonia shinshuensis DB 102 ( T ) , L. poae VKM Ac-1401 ( T ) , L. naganoensis DB 103 ( T ) , L. aquatica DSM 20146 ( T ) and L. xyli subsp .
	manualset3
97488	7	400888	13	NULL	NULL	0	NULL	L. naganoensis DB 103 ( T )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	16S rRNA gene sequence analysis of strain TG-S248 ( T ) with sequences from Leifsonia shinshuensis DB 102 ( T ) , L. poae VKM Ac-1401 ( T ) , L. naganoensis DB 103 ( T ) , L. aquatica DSM 20146 ( T ) and L. xyli subsp .
	manualset3
97489	8	400888	13	NULL	NULL	0	NULL	L. aquatica DSM 20146 ( T ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	16S rRNA gene sequence analysis of strain TG-S248 ( T ) with sequences from Leifsonia shinshuensis DB 102 ( T ) , L. poae VKM Ac-1401 ( T ) , L. naganoensis DB 103 ( T ) , L. aquatica DSM 20146 ( T ) and L. xyli subsp .
	manualset3
97490	9	400888	13	NULL	NULL	0	NULL	L. xyli subsp 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	16S rRNA gene sequence analysis of strain TG-S248 ( T ) with sequences from Leifsonia shinshuensis DB 102 ( T ) , L. poae VKM Ac-1401 ( T ) , L. naganoensis DB 103 ( T ) , L. aquatica DSM 20146 ( T ) and L. xyli subsp .
	manualset3
97491	1	400889	13	NULL	NULL	0	NULL	respect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , a preliminary analysis of TCR utilization in three T cell clones specific for MBP 68-88 isolated from animals recovered from active EAE indicates that while all three use V beta 8.2 , only one contains AspSer in the CDR3 .
	manualset3
97492	2	400889	13	NULL	NULL	0	NULL	preliminary analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , a preliminary analysis of TCR utilization in three T cell clones specific for MBP 68-88 isolated from animals recovered from active EAE indicates that while all three use V beta 8.2 , only one contains AspSer in the CDR3 .
	manualset3
97493	3	400889	13	NULL	NULL	0	NULL	TCR utilization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , a preliminary analysis of TCR utilization in three T cell clones specific for MBP 68-88 isolated from animals recovered from active EAE indicates that while all three use V beta 8.2 , only one contains AspSer in the CDR3 .
	manualset3
97494	4	400889	13	NULL	NULL	0	NULL	three 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , a preliminary analysis of TCR utilization in three T cell clones specific for MBP 68-88 isolated from animals recovered from active EAE indicates that while all three use V beta 8.2 , only one contains AspSer in the CDR3 .
	manualset3
97495	5	400889	13	NULL	NULL	0	NULL	T cell clones	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , a preliminary analysis of TCR utilization in three T cell clones specific for MBP 68-88 isolated from animals recovered from active EAE indicates that while all three use V beta 8.2 , only one contains AspSer in the CDR3 .
	manualset3
97496	6	400889	13	NULL	NULL	0	NULL	MBP 68-88 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , a preliminary analysis of TCR utilization in three T cell clones specific for MBP 68-88 isolated from animals recovered from active EAE indicates that while all three use V beta 8.2 , only one contains AspSer in the CDR3 .
	manualset3
97497	7	400889	13	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , a preliminary analysis of TCR utilization in three T cell clones specific for MBP 68-88 isolated from animals recovered from active EAE indicates that while all three use V beta 8.2 , only one contains AspSer in the CDR3 .
	manualset3
97498	8	400889	13	NULL	NULL	0	NULL	 EAE	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , a preliminary analysis of TCR utilization in three T cell clones specific for MBP 68-88 isolated from animals recovered from active EAE indicates that while all three use V beta 8.2 , only one contains AspSer in the CDR3 .
	manualset3
97499	9	400889	13	NULL	NULL	0	NULL	three 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , a preliminary analysis of TCR utilization in three T cell clones specific for MBP 68-88 isolated from animals recovered from active EAE indicates that while all three use V beta 8.2 , only one contains AspSer in the CDR3 .
	manualset3
97500	10	400889	13	NULL	NULL	NULL	NULL	V beta 8.2 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this respect , a preliminary analysis of TCR utilization in three T cell clones specific for MBP 68-88 isolated from animals recovered from active EAE indicates that while all three use V beta 8.2 , only one contains AspSer in the CDR3 .
	manualset3
97501	11	400889	13	NULL	NULL	0	NULL	AspSer	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , a preliminary analysis of TCR utilization in three T cell clones specific for MBP 68-88 isolated from animals recovered from active EAE indicates that while all three use V beta 8.2 , only one contains AspSer in the CDR3 .
	manualset3
97502	12	400889	13	NULL	NULL	0	NULL	CDR3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , a preliminary analysis of TCR utilization in three T cell clones specific for MBP 68-88 isolated from animals recovered from active EAE indicates that while all three use V beta 8.2 , only one contains AspSer in the CDR3 .
	manualset3
97503	1	400890	13	NULL	NULL	0	NULL	respect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , economic forces are nudging both systems towards a convergence of structure and performance .
	manualset3
97504	2	400890	13	NULL	NULL	0	NULL	economic forces 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , economic forces are nudging both systems towards a convergence of structure and performance .
	manualset3
97505	3	400890	13	NULL	NULL	NULL	NULL	systems	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this respect , economic forces are nudging both systems towards a convergence of structure and performance .
	manualset3
97506	4	400890	13	NULL	NULL	0	NULL	convergence of structure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , economic forces are nudging both systems towards a convergence of structure and performance .
	manualset3
97507	5	400890	13	NULL	NULL	0	NULL	performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , economic forces are nudging both systems towards a convergence of structure and performance .
	manualset3
97508	1	400891	13	NULL	NULL	0	NULL	 respect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , galactofuranose-based glycoconjugates are interesting target molecules for drug design .
	manualset3
97509	2	400891	13	NULL	NULL	0	NULL	galactofuranose-based glycoconjugates	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , galactofuranose-based glycoconjugates are interesting target molecules for drug design .
	manualset3
97510	3	400891	13	NULL	NULL	0	NULL	target molecules	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , galactofuranose-based glycoconjugates are interesting target molecules for drug design .
	manualset3
97511	4	400891	13	NULL	NULL	0	NULL	drug design	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , galactofuranose-based glycoconjugates are interesting target molecules for drug design .
	manualset3
97512	1	400892	13	NULL	NULL	0	NULL	respect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , one of the largest water technology projects worldwide is the Yangtze Three Gorges Dam in China .
	manualset3
97513	2	400892	13	NULL	NULL	0	NULL	water technology projects	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , one of the largest water technology projects worldwide is the Yangtze Three Gorges Dam in China .
	manualset3
97514	3	400892	13	NULL	NULL	0	NULL	Yangtze Three Gorges Dam	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , one of the largest water technology projects worldwide is the Yangtze Three Gorges Dam in China .
	manualset3
97515	4	400892	13	NULL	NULL	0	NULL	China	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , one of the largest water technology projects worldwide is the Yangtze Three Gorges Dam in China .
	manualset3
97516	1	400893	13	NULL	NULL	0	NULL	review 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , the ability of these models to account for the binding of nicotinic agents at alpha4beta2 nACh receptors ( or rat brain receptors for which alpha4beta2 receptors are the major component ) is assessed .
	manualset3
97517	2	400893	13	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , the ability of these models to account for the binding of nicotinic agents at alpha4beta2 nACh receptors ( or rat brain receptors for which alpha4beta2 receptors are the major component ) is assessed .
	manualset3
97518	3	400893	13	NULL	NULL	0	NULL	models 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , the ability of these models to account for the binding of nicotinic agents at alpha4beta2 nACh receptors ( or rat brain receptors for which alpha4beta2 receptors are the major component ) is assessed .
	manualset3
97519	4	400893	13	NULL	NULL	0	NULL	binding of nicotinic agents at alpha4beta2 nACh receptors 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , the ability of these models to account for the binding of nicotinic agents at alpha4beta2 nACh receptors ( or rat brain receptors for which alpha4beta2 receptors are the major component ) is assessed .
	manualset3
97520	5	400893	13	NULL	NULL	0	NULL	rat brain receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , the ability of these models to account for the binding of nicotinic agents at alpha4beta2 nACh receptors ( or rat brain receptors for which alpha4beta2 receptors are the major component ) is assessed .
	manualset3
97521	6	400893	13	NULL	NULL	0	NULL	alpha4beta2 receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , the ability of these models to account for the binding of nicotinic agents at alpha4beta2 nACh receptors ( or rat brain receptors for which alpha4beta2 receptors are the major component ) is assessed .
	manualset3
97522	7	400893	13	NULL	NULL	0	NULL	major component	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , the ability of these models to account for the binding of nicotinic agents at alpha4beta2 nACh receptors ( or rat brain receptors for which alpha4beta2 receptors are the major component ) is assessed .
	manualset3
97523	1	400894	13	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we bring together recent studies investigating STDP in neurodevelopmental learning disorders using Fragile X syndrome as a model and we argue that alterations in dendritic excitability underlie deficits seen in STDP .
	manualset3
97524	2	400894	13	NULL	NULL	0	NULL	recent studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we bring together recent studies investigating STDP in neurodevelopmental learning disorders using Fragile X syndrome as a model and we argue that alterations in dendritic excitability underlie deficits seen in STDP .
	manualset3
97525	3	400894	13	NULL	NULL	0	NULL	STDP	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we bring together recent studies investigating STDP in neurodevelopmental learning disorders using Fragile X syndrome as a model and we argue that alterations in dendritic excitability underlie deficits seen in STDP .
	manualset3
97526	4	400894	13	NULL	NULL	NULL	NULL	neurodevelopmental learning disorders	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this review , we bring together recent studies investigating STDP in neurodevelopmental learning disorders using Fragile X syndrome as a model and we argue that alterations in dendritic excitability underlie deficits seen in STDP .
	manualset3
97527	5	400894	13	NULL	NULL	0	NULL	Fragile X syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we bring together recent studies investigating STDP in neurodevelopmental learning disorders using Fragile X syndrome as a model and we argue that alterations in dendritic excitability underlie deficits seen in STDP .
	manualset3
97528	6	400894	13	NULL	NULL	0	NULL	model	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we bring together recent studies investigating STDP in neurodevelopmental learning disorders using Fragile X syndrome as a model and we argue that alterations in dendritic excitability underlie deficits seen in STDP .
	manualset3
97529	7	400894	13	NULL	NULL	0	NULL	alterations in dendritic excitability 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we bring together recent studies investigating STDP in neurodevelopmental learning disorders using Fragile X syndrome as a model and we argue that alterations in dendritic excitability underlie deficits seen in STDP .
	manualset3
97530	8	400894	13	NULL	NULL	0	NULL	deficits 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we bring together recent studies investigating STDP in neurodevelopmental learning disorders using Fragile X syndrome as a model and we argue that alterations in dendritic excitability underlie deficits seen in STDP .
	manualset3
97531	9	400894	13	NULL	NULL	0	NULL	 STDP	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we bring together recent studies investigating STDP in neurodevelopmental learning disorders using Fragile X syndrome as a model and we argue that alterations in dendritic excitability underlie deficits seen in STDP .
	manualset3
97532	1	400895	13	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we delineate oxidative protein modifications existing in diabetic nephropathy and discuss therapeutic perspectives towards the development of new classes of renoprotective agents .
	manualset3
97533	2	400895	13	NULL	NULL	0	NULL	 oxidative protein modifications	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we delineate oxidative protein modifications existing in diabetic nephropathy and discuss therapeutic perspectives towards the development of new classes of renoprotective agents .
	manualset3
97534	3	400895	13	NULL	NULL	0	NULL	diabetic nephropathy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we delineate oxidative protein modifications existing in diabetic nephropathy and discuss therapeutic perspectives towards the development of new classes of renoprotective agents .
	manualset3
97535	4	400895	13	NULL	NULL	0	NULL	therapeutic perspectives	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we delineate oxidative protein modifications existing in diabetic nephropathy and discuss therapeutic perspectives towards the development of new classes of renoprotective agents .
	manualset3
97536	5	400895	13	NULL	NULL	0	NULL	 development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we delineate oxidative protein modifications existing in diabetic nephropathy and discuss therapeutic perspectives towards the development of new classes of renoprotective agents .
	manualset3
97537	6	400895	13	NULL	NULL	0	NULL	new classes of renoprotective agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we delineate oxidative protein modifications existing in diabetic nephropathy and discuss therapeutic perspectives towards the development of new classes of renoprotective agents .
	manualset3
97538	1	400896	13	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we describe the role of the Bcl-2 protein family , and to a lesser extent that of death receptors ( members of the tumor necrosis factor receptor family with a death domain ) , in the control of lymphoid and myeloid cell survival .
	manualset3
97539	2	400896	13	NULL	NULL	0	NULL	 role 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we describe the role of the Bcl-2 protein family , and to a lesser extent that of death receptors ( members of the tumor necrosis factor receptor family with a death domain ) , in the control of lymphoid and myeloid cell survival .
	manualset3
97540	3	400896	13	NULL	NULL	0	NULL	Bcl-2 protein family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we describe the role of the Bcl-2 protein family , and to a lesser extent that of death receptors ( members of the tumor necrosis factor receptor family with a death domain ) , in the control of lymphoid and myeloid cell survival .
	manualset3
97541	4	400896	13	NULL	NULL	0	NULL	death receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we describe the role of the Bcl-2 protein family , and to a lesser extent that of death receptors ( members of the tumor necrosis factor receptor family with a death domain ) , in the control of lymphoid and myeloid cell survival .
	manualset3
97542	5	400896	13	NULL	NULL	0	NULL	 members of the tumor necrosis factor receptor family with a death domain	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we describe the role of the Bcl-2 protein family , and to a lesser extent that of death receptors ( members of the tumor necrosis factor receptor family with a death domain ) , in the control of lymphoid and myeloid cell survival .
	manualset3
97543	6	400896	13	NULL	NULL	0	NULL	control	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we describe the role of the Bcl-2 protein family , and to a lesser extent that of death receptors ( members of the tumor necrosis factor receptor family with a death domain ) , in the control of lymphoid and myeloid cell survival .
	manualset3
97544	7	400896	13	NULL	NULL	0	NULL	 lymphoid cell survival 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we describe the role of the Bcl-2 protein family , and to a lesser extent that of death receptors ( members of the tumor necrosis factor receptor family with a death domain ) , in the control of lymphoid and myeloid cell survival .
	manualset3
97545	8	400896	13	NULL	NULL	0	NULL	myeloid cell survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we describe the role of the Bcl-2 protein family , and to a lesser extent that of death receptors ( members of the tumor necrosis factor receptor family with a death domain ) , in the control of lymphoid and myeloid cell survival .
	manualset3
97546	1	400897	13	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss sex differences in EDHF biology and how sex hormones can modulate EDHF responses .
	manualset3
97547	2	400897	13	NULL	NULL	0	NULL	sex differences 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss sex differences in EDHF biology and how sex hormones can modulate EDHF responses .
	manualset3
97548	3	400897	13	NULL	NULL	0	NULL	 EDHF biology 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss sex differences in EDHF biology and how sex hormones can modulate EDHF responses .
	manualset3
97549	4	400897	13	NULL	NULL	0	NULL	sex hormones	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss sex differences in EDHF biology and how sex hormones can modulate EDHF responses .
	manualset3
97550	5	400897	13	NULL	NULL	0	NULL	EDHF responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss sex differences in EDHF biology and how sex hormones can modulate EDHF responses .
	manualset3
97551	1	400898	13	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss the ample evidence focused on the roles of TLRs and CD4 ( + ) helper T cell subsets on the progression of acute viral encephalitis .
	manualset3
97552	2	400898	13	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss the ample evidence focused on the roles of TLRs and CD4 ( + ) helper T cell subsets on the progression of acute viral encephalitis .
	manualset3
97553	3	400898	13	NULL	NULL	0	NULL	 roles 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss the ample evidence focused on the roles of TLRs and CD4 ( + ) helper T cell subsets on the progression of acute viral encephalitis .
	manualset3
97554	4	400898	13	NULL	NULL	0	NULL	TLRs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss the ample evidence focused on the roles of TLRs and CD4 ( + ) helper T cell subsets on the progression of acute viral encephalitis .
	manualset3
97555	5	400898	13	NULL	NULL	0	NULL	CD4 ( + ) helper T cell subsets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss the ample evidence focused on the roles of TLRs and CD4 ( + ) helper T cell subsets on the progression of acute viral encephalitis .
	manualset3
97556	6	400898	13	NULL	NULL	0	NULL	progression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss the ample evidence focused on the roles of TLRs and CD4 ( + ) helper T cell subsets on the progression of acute viral encephalitis .
	manualset3
97557	7	400898	13	NULL	NULL	0	NULL	acute viral encephalitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss the ample evidence focused on the roles of TLRs and CD4 ( + ) helper T cell subsets on the progression of acute viral encephalitis .
	manualset3
97558	1	400899	13	NULL	NULL	NULL	NULL	17alpha-Hydroxyandrost-4-en-3-one	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	17alpha-Hydroxyandrost-4-en-3-one and 3beta , 17alpha-dihydroxypregn-5-en-20-one were considered as possible precursors for androst-16-ene formation , but both were shown to be ineffective .
	manualset3
97559	2	400899	13	NULL	NULL	NULL	NULL	3beta , 17alpha-dihydroxypregn-5-en-20-one	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	17alpha-Hydroxyandrost-4-en-3-one and 3beta , 17alpha-dihydroxypregn-5-en-20-one were considered as possible precursors for androst-16-ene formation , but both were shown to be ineffective .
	manualset3
97560	3	400899	13	NULL	NULL	NULL	NULL	 precursors	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	17alpha-Hydroxyandrost-4-en-3-one and 3beta , 17alpha-dihydroxypregn-5-en-20-one were considered as possible precursors for androst-16-ene formation , but both were shown to be ineffective .
	manualset3
97561	4	400899	13	NULL	NULL	NULL	NULL	androst-16-ene formation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	17alpha-Hydroxyandrost-4-en-3-one and 3beta , 17alpha-dihydroxypregn-5-en-20-one were considered as possible precursors for androst-16-ene formation , but both were shown to be ineffective .
	manualset3
97578	1	400900	13	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss the importance of , and requirements for , effective interactions between B cells and T cells during the formation of CD4 ( + ) T follicular helper cells and the elicitation of cytotoxic function of virus-specific CD8 ( + ) T cells , as well as how these processes are abrogated in primary immunodeficiencies due to loss-of-function mutations in defined genes .
	manualset3
97579	2	400900	13	NULL	NULL	0	NULL	importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss the importance of , and requirements for , effective interactions between B cells and T cells during the formation of CD4 ( + ) T follicular helper cells and the elicitation of cytotoxic function of virus-specific CD8 ( + ) T cells , as well as how these processes are abrogated in primary immunodeficiencies due to loss-of-function mutations in defined genes .
	manualset3
97580	3	400900	13	NULL	NULL	0	NULL	requirements 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss the importance of , and requirements for , effective interactions between B cells and T cells during the formation of CD4 ( + ) T follicular helper cells and the elicitation of cytotoxic function of virus-specific CD8 ( + ) T cells , as well as how these processes are abrogated in primary immunodeficiencies due to loss-of-function mutations in defined genes .
	manualset3
97581	4	400900	13	NULL	NULL	0	NULL	 interactions 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss the importance of , and requirements for , effective interactions between B cells and T cells during the formation of CD4 ( + ) T follicular helper cells and the elicitation of cytotoxic function of virus-specific CD8 ( + ) T cells , as well as how these processes are abrogated in primary immunodeficiencies due to loss-of-function mutations in defined genes .
	manualset3
97582	5	400900	13	NULL	NULL	0	NULL	B cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss the importance of , and requirements for , effective interactions between B cells and T cells during the formation of CD4 ( + ) T follicular helper cells and the elicitation of cytotoxic function of virus-specific CD8 ( + ) T cells , as well as how these processes are abrogated in primary immunodeficiencies due to loss-of-function mutations in defined genes .
	manualset3
97583	6	400900	13	NULL	NULL	0	NULL	T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss the importance of , and requirements for , effective interactions between B cells and T cells during the formation of CD4 ( + ) T follicular helper cells and the elicitation of cytotoxic function of virus-specific CD8 ( + ) T cells , as well as how these processes are abrogated in primary immunodeficiencies due to loss-of-function mutations in defined genes .
	manualset3
97584	7	400900	13	NULL	NULL	0	NULL	formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss the importance of , and requirements for , effective interactions between B cells and T cells during the formation of CD4 ( + ) T follicular helper cells and the elicitation of cytotoxic function of virus-specific CD8 ( + ) T cells , as well as how these processes are abrogated in primary immunodeficiencies due to loss-of-function mutations in defined genes .
	manualset3
97585	8	400900	13	NULL	NULL	0	NULL	CD4 ( + ) T follicular helper cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss the importance of , and requirements for , effective interactions between B cells and T cells during the formation of CD4 ( + ) T follicular helper cells and the elicitation of cytotoxic function of virus-specific CD8 ( + ) T cells , as well as how these processes are abrogated in primary immunodeficiencies due to loss-of-function mutations in defined genes .
	manualset3
97586	9	400900	13	NULL	NULL	0	NULL	elicitation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss the importance of , and requirements for , effective interactions between B cells and T cells during the formation of CD4 ( + ) T follicular helper cells and the elicitation of cytotoxic function of virus-specific CD8 ( + ) T cells , as well as how these processes are abrogated in primary immunodeficiencies due to loss-of-function mutations in defined genes .
	manualset3
97587	10	400900	13	NULL	NULL	0	NULL	cytotoxic function 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss the importance of , and requirements for , effective interactions between B cells and T cells during the formation of CD4 ( + ) T follicular helper cells and the elicitation of cytotoxic function of virus-specific CD8 ( + ) T cells , as well as how these processes are abrogated in primary immunodeficiencies due to loss-of-function mutations in defined genes .
	manualset3
97588	11	400900	13	NULL	NULL	0	NULL	virus-specific CD8 ( + ) T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss the importance of , and requirements for , effective interactions between B cells and T cells during the formation of CD4 ( + ) T follicular helper cells and the elicitation of cytotoxic function of virus-specific CD8 ( + ) T cells , as well as how these processes are abrogated in primary immunodeficiencies due to loss-of-function mutations in defined genes .
	manualset3
97589	12	400900	13	NULL	NULL	0	NULL	 processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss the importance of , and requirements for , effective interactions between B cells and T cells during the formation of CD4 ( + ) T follicular helper cells and the elicitation of cytotoxic function of virus-specific CD8 ( + ) T cells , as well as how these processes are abrogated in primary immunodeficiencies due to loss-of-function mutations in defined genes .
	manualset3
97590	13	400900	13	NULL	NULL	0	NULL	immunodeficiencies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss the importance of , and requirements for , effective interactions between B cells and T cells during the formation of CD4 ( + ) T follicular helper cells and the elicitation of cytotoxic function of virus-specific CD8 ( + ) T cells , as well as how these processes are abrogated in primary immunodeficiencies due to loss-of-function mutations in defined genes .
	manualset3
97591	14	400900	13	NULL	NULL	NULL	NULL	loss-of-function mutations	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this review , we discuss the importance of , and requirements for , effective interactions between B cells and T cells during the formation of CD4 ( + ) T follicular helper cells and the elicitation of cytotoxic function of virus-specific CD8 ( + ) T cells , as well as how these processes are abrogated in primary immunodeficiencies due to loss-of-function mutations in defined genes .
	manualset3
97592	15	400900	13	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss the importance of , and requirements for , effective interactions between B cells and T cells during the formation of CD4 ( + ) T follicular helper cells and the elicitation of cytotoxic function of virus-specific CD8 ( + ) T cells , as well as how these processes are abrogated in primary immunodeficiencies due to loss-of-function mutations in defined genes .
	manualset3
97593	1	400901	13	NULL	NULL	0	NULL	 review 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we examine what is known about NeuroD and what remains to be answered .
	manualset3
97594	2	400901	13	NULL	NULL	0	NULL	NeuroD	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we examine what is known about NeuroD and what remains to be answered .
	manualset3
97595	1	400902	13	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we focus on new functions of platelets that may be involved in the host response to infection .
	manualset3
97596	2	400902	13	NULL	NULL	0	NULL	focus 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we focus on new functions of platelets that may be involved in the host response to infection .
	manualset3
97597	3	400902	13	NULL	NULL	0	NULL	functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we focus on new functions of platelets that may be involved in the host response to infection .
	manualset3
97598	4	400902	13	NULL	NULL	0	NULL	platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we focus on new functions of platelets that may be involved in the host response to infection .
	manualset3
97599	5	400902	13	NULL	NULL	0	NULL	host response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we focus on new functions of platelets that may be involved in the host response to infection .
	manualset3
97600	6	400902	13	NULL	NULL	0	NULL	infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we focus on new functions of platelets that may be involved in the host response to infection .
	manualset3
97601	1	400903	13	NULL	NULL	0	NULL	 review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we highlight recent advances and caveats relating to the application of this powerful new methodology to hematopoiesis .
	manualset3
97602	2	400903	13	NULL	NULL	0	NULL	highlight recent advances	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we highlight recent advances and caveats relating to the application of this powerful new methodology to hematopoiesis .
	manualset3
97603	3	400903	13	NULL	NULL	0	NULL	 caveats	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we highlight recent advances and caveats relating to the application of this powerful new methodology to hematopoiesis .
	manualset3
97604	4	400903	13	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we highlight recent advances and caveats relating to the application of this powerful new methodology to hematopoiesis .
	manualset3
97605	5	400903	13	NULL	NULL	0	NULL	methodology	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we highlight recent advances and caveats relating to the application of this powerful new methodology to hematopoiesis .
	manualset3
97606	6	400903	13	NULL	NULL	0	NULL	hematopoiesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we highlight recent advances and caveats relating to the application of this powerful new methodology to hematopoiesis .
	manualset3
97607	1	400904	13	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we summarize the latest clinical and scientific information on these metabolic complications , examine current hypotheses explaining the syndromes and comment on the existing methods available to manage these metabolic side effects .
	manualset3
97608	2	400904	13	NULL	NULL	0	NULL	clinical information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we summarize the latest clinical and scientific information on these metabolic complications , examine current hypotheses explaining the syndromes and comment on the existing methods available to manage these metabolic side effects .
	manualset3
97609	3	400904	13	NULL	NULL	0	NULL	scientific information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we summarize the latest clinical and scientific information on these metabolic complications , examine current hypotheses explaining the syndromes and comment on the existing methods available to manage these metabolic side effects .
	manualset3
97610	4	400904	13	NULL	NULL	0	NULL	metabolic complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we summarize the latest clinical and scientific information on these metabolic complications , examine current hypotheses explaining the syndromes and comment on the existing methods available to manage these metabolic side effects .
	manualset3
97611	5	400904	13	NULL	NULL	0	NULL	 current hypotheses 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we summarize the latest clinical and scientific information on these metabolic complications , examine current hypotheses explaining the syndromes and comment on the existing methods available to manage these metabolic side effects .
	manualset3
97612	6	400904	13	NULL	NULL	0	NULL	 syndromes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we summarize the latest clinical and scientific information on these metabolic complications , examine current hypotheses explaining the syndromes and comment on the existing methods available to manage these metabolic side effects .
	manualset3
97613	7	400904	13	NULL	NULL	0	NULL	comment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we summarize the latest clinical and scientific information on these metabolic complications , examine current hypotheses explaining the syndromes and comment on the existing methods available to manage these metabolic side effects .
	manualset3
97614	8	400904	13	NULL	NULL	0	NULL	methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we summarize the latest clinical and scientific information on these metabolic complications , examine current hypotheses explaining the syndromes and comment on the existing methods available to manage these metabolic side effects .
	manualset3
97615	9	400904	13	NULL	NULL	0	NULL	metabolic side effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we summarize the latest clinical and scientific information on these metabolic complications , examine current hypotheses explaining the syndromes and comment on the existing methods available to manage these metabolic side effects .
	manualset3
97616	1	400905	13	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we will describe the molecular mechanisms of actions of one , GRIM-19 , which participates in multiple pathways for exerting growth control and/or cell death .
	manualset3
97617	2	400905	13	NULL	NULL	NULL	NULL	molecular mechanisms of actions 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this review , we will describe the molecular mechanisms of actions of one , GRIM-19 , which participates in multiple pathways for exerting growth control and/or cell death .
	manualset3
97618	3	400905	13	NULL	NULL	0	NULL	GRIM-19	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we will describe the molecular mechanisms of actions of one , GRIM-19 , which participates in multiple pathways for exerting growth control and/or cell death .
	manualset3
97619	4	400905	13	NULL	NULL	0	NULL	multiple pathways 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we will describe the molecular mechanisms of actions of one , GRIM-19 , which participates in multiple pathways for exerting growth control and/or cell death .
	manualset3
97620	5	400905	13	NULL	NULL	0	NULL	growth control 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we will describe the molecular mechanisms of actions of one , GRIM-19 , which participates in multiple pathways for exerting growth control and/or cell death .
	manualset3
97621	6	400905	13	NULL	NULL	0	NULL	cell death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we will describe the molecular mechanisms of actions of one , GRIM-19 , which participates in multiple pathways for exerting growth control and/or cell death .
	manualset3
97622	1	400906	13	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , what has been learned about health professional/patient communication and patient education ( skills , settings and materials ) , lay and health professional liaison ( including telephone helplines ) , patient education in low-income countries , the integration of patient education into clinical practice , health professional training and the implementation of guidelines , and the role of national asthma campaigns is drawn together .
	manualset3
97623	2	400906	13	NULL	NULL	0	NULL	health professional/patient communication 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , what has been learned about health professional/patient communication and patient education ( skills , settings and materials ) , lay and health professional liaison ( including telephone helplines ) , patient education in low-income countries , the integration of patient education into clinical practice , health professional training and the implementation of guidelines , and the role of national asthma campaigns is drawn together .
	manualset3
97624	3	400906	13	NULL	NULL	0	NULL	patient education ( skills , settings and materials )	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , what has been learned about health professional/patient communication and patient education ( skills , settings and materials ) , lay and health professional liaison ( including telephone helplines ) , patient education in low-income countries , the integration of patient education into clinical practice , health professional training and the implementation of guidelines , and the role of national asthma campaigns is drawn together .
	manualset3
97625	4	400906	13	NULL	NULL	0	NULL	 health professional liaison	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , what has been learned about health professional/patient communication and patient education ( skills , settings and materials ) , lay and health professional liaison ( including telephone helplines ) , patient education in low-income countries , the integration of patient education into clinical practice , health professional training and the implementation of guidelines , and the role of national asthma campaigns is drawn together .
	manualset3
97626	5	400906	13	NULL	NULL	0	NULL	telephone helplines	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , what has been learned about health professional/patient communication and patient education ( skills , settings and materials ) , lay and health professional liaison ( including telephone helplines ) , patient education in low-income countries , the integration of patient education into clinical practice , health professional training and the implementation of guidelines , and the role of national asthma campaigns is drawn together .
	manualset3
97627	6	400906	13	NULL	NULL	0	NULL	patient education	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , what has been learned about health professional/patient communication and patient education ( skills , settings and materials ) , lay and health professional liaison ( including telephone helplines ) , patient education in low-income countries , the integration of patient education into clinical practice , health professional training and the implementation of guidelines , and the role of national asthma campaigns is drawn together .
	manualset3
97628	7	400906	13	NULL	NULL	0	NULL	low-income countries	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , what has been learned about health professional/patient communication and patient education ( skills , settings and materials ) , lay and health professional liaison ( including telephone helplines ) , patient education in low-income countries , the integration of patient education into clinical practice , health professional training and the implementation of guidelines , and the role of national asthma campaigns is drawn together .
	manualset3
97629	8	400906	13	NULL	NULL	0	NULL	integration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , what has been learned about health professional/patient communication and patient education ( skills , settings and materials ) , lay and health professional liaison ( including telephone helplines ) , patient education in low-income countries , the integration of patient education into clinical practice , health professional training and the implementation of guidelines , and the role of national asthma campaigns is drawn together .
	manualset3
97630	9	400906	13	NULL	NULL	0	NULL	patient education	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , what has been learned about health professional/patient communication and patient education ( skills , settings and materials ) , lay and health professional liaison ( including telephone helplines ) , patient education in low-income countries , the integration of patient education into clinical practice , health professional training and the implementation of guidelines , and the role of national asthma campaigns is drawn together .
	manualset3
97631	10	400906	13	NULL	NULL	0	NULL	clinical practice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , what has been learned about health professional/patient communication and patient education ( skills , settings and materials ) , lay and health professional liaison ( including telephone helplines ) , patient education in low-income countries , the integration of patient education into clinical practice , health professional training and the implementation of guidelines , and the role of national asthma campaigns is drawn together .
	manualset3
97632	11	400906	13	NULL	NULL	0	NULL	health professional training 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , what has been learned about health professional/patient communication and patient education ( skills , settings and materials ) , lay and health professional liaison ( including telephone helplines ) , patient education in low-income countries , the integration of patient education into clinical practice , health professional training and the implementation of guidelines , and the role of national asthma campaigns is drawn together .
	manualset3
97633	12	400906	13	NULL	NULL	0	NULL	implementation of guidelines	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , what has been learned about health professional/patient communication and patient education ( skills , settings and materials ) , lay and health professional liaison ( including telephone helplines ) , patient education in low-income countries , the integration of patient education into clinical practice , health professional training and the implementation of guidelines , and the role of national asthma campaigns is drawn together .
	manualset3
97634	13	400906	13	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , what has been learned about health professional/patient communication and patient education ( skills , settings and materials ) , lay and health professional liaison ( including telephone helplines ) , patient education in low-income countries , the integration of patient education into clinical practice , health professional training and the implementation of guidelines , and the role of national asthma campaigns is drawn together .
	manualset3
97635	14	400906	13	NULL	NULL	0	NULL	national asthma campaigns	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , what has been learned about health professional/patient communication and patient education ( skills , settings and materials ) , lay and health professional liaison ( including telephone helplines ) , patient education in low-income countries , the integration of patient education into clinical practice , health professional training and the implementation of guidelines , and the role of national asthma campaigns is drawn together .
	manualset3
97636	1	400907	13	NULL	NULL	0	NULL	17alpha-oestradiol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	17alpha-oestradiol also inhibited the current , but with a maximal inhibition of only 17 % .
	manualset3
97637	2	400907	13	NULL	NULL	0	NULL	 inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	17alpha-oestradiol also inhibited the current , but with a maximal inhibition of only 17 % .
	manualset3
97638	3	400907	13	NULL	NULL	0	NULL	17 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	17alpha-oestradiol also inhibited the current , but with a maximal inhibition of only 17 % .
	manualset3
97639	1	400908	13	NULL	NULL	0	NULL	review article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review article , clinical findings of liver involvement in HHT and their pathophysiology are discussed as well as diagnostic methodologies , therapies used and their outcome .
	manualset3
97640	2	400908	13	NULL	NULL	0	NULL	clinical findings	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review article , clinical findings of liver involvement in HHT and their pathophysiology are discussed as well as diagnostic methodologies , therapies used and their outcome .
	manualset3
97641	3	400908	13	NULL	NULL	0	NULL	 liver 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review article , clinical findings of liver involvement in HHT and their pathophysiology are discussed as well as diagnostic methodologies , therapies used and their outcome .
	manualset3
97642	4	400908	13	NULL	NULL	0	NULL	 involvement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review article , clinical findings of liver involvement in HHT and their pathophysiology are discussed as well as diagnostic methodologies , therapies used and their outcome .
	manualset3
97643	5	400908	13	NULL	NULL	0	NULL	HHT	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review article , clinical findings of liver involvement in HHT and their pathophysiology are discussed as well as diagnostic methodologies , therapies used and their outcome .
	manualset3
97644	6	400908	13	NULL	NULL	0	NULL	pathophysiology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review article , clinical findings of liver involvement in HHT and their pathophysiology are discussed as well as diagnostic methodologies , therapies used and their outcome .
	manualset3
97645	7	400908	13	NULL	NULL	0	NULL	diagnostic methodologies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review article , clinical findings of liver involvement in HHT and their pathophysiology are discussed as well as diagnostic methodologies , therapies used and their outcome .
	manualset3
97646	8	400908	13	NULL	NULL	0	NULL	therapies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review article , clinical findings of liver involvement in HHT and their pathophysiology are discussed as well as diagnostic methodologies , therapies used and their outcome .
	manualset3
97647	9	400908	13	NULL	NULL	0	NULL	outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review article , clinical findings of liver involvement in HHT and their pathophysiology are discussed as well as diagnostic methodologies , therapies used and their outcome .
	manualset3
97648	1	400909	13	NULL	NULL	0	NULL	review 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review structure-activity relationships of morphiceptin analogs and studies resulting in defining low energy conformations are discussed .
	manualset3
97649	2	400909	13	NULL	NULL	0	NULL	structure-activity relationships	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review structure-activity relationships of morphiceptin analogs and studies resulting in defining low energy conformations are discussed .
	manualset3
97650	3	400909	13	NULL	NULL	0	NULL	 morphiceptin analogs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review structure-activity relationships of morphiceptin analogs and studies resulting in defining low energy conformations are discussed .
	manualset3
97651	4	400909	13	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review structure-activity relationships of morphiceptin analogs and studies resulting in defining low energy conformations are discussed .
	manualset3
97652	1	400910	13	NULL	NULL	NULL	NULL	review 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this review we deal with the importance of properties such as fimbriae and adhesins as well as systems to meet the bacterial need for iron during infection .
	manualset3
97653	2	400910	13	NULL	NULL	0	NULL	importance of properties	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review we deal with the importance of properties such as fimbriae and adhesins as well as systems to meet the bacterial need for iron during infection .
	manualset3
97654	3	400910	13	NULL	NULL	NULL	NULL	fimbriae	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this review we deal with the importance of properties such as fimbriae and adhesins as well as systems to meet the bacterial need for iron during infection .
	manualset3
97655	4	400910	13	NULL	NULL	0	NULL	adhesins	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review we deal with the importance of properties such as fimbriae and adhesins as well as systems to meet the bacterial need for iron during infection .
	manualset3
97656	5	400910	13	NULL	NULL	0	NULL	systems	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review we deal with the importance of properties such as fimbriae and adhesins as well as systems to meet the bacterial need for iron during infection .
	manualset3
97657	6	400910	13	NULL	NULL	NULL	NULL	bacterial need	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this review we deal with the importance of properties such as fimbriae and adhesins as well as systems to meet the bacterial need for iron during infection .
	manualset3
97658	7	400910	13	NULL	NULL	NULL	NULL	iron	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this review we deal with the importance of properties such as fimbriae and adhesins as well as systems to meet the bacterial need for iron during infection .
	manualset3
97659	8	400910	13	NULL	NULL	0	NULL	infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review we deal with the importance of properties such as fimbriae and adhesins as well as systems to meet the bacterial need for iron during infection .
	manualset3
97660	1	400911	13	NULL	NULL	0	NULL	review 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review we focus our attention on cellular ROS level to trigger beneficial effects on plant cells responding to pathogen attack .
	manualset3
97661	2	400911	13	NULL	NULL	0	NULL	focus 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review we focus our attention on cellular ROS level to trigger beneficial effects on plant cells responding to pathogen attack .
	manualset3
97662	3	400911	13	NULL	NULL	0	NULL	 attention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review we focus our attention on cellular ROS level to trigger beneficial effects on plant cells responding to pathogen attack .
	manualset3
97663	4	400911	13	NULL	NULL	0	NULL	cellular ROS level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review we focus our attention on cellular ROS level to trigger beneficial effects on plant cells responding to pathogen attack .
	manualset3
97664	5	400911	13	NULL	NULL	0	NULL	beneficial effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review we focus our attention on cellular ROS level to trigger beneficial effects on plant cells responding to pathogen attack .
	manualset3
97665	6	400911	13	NULL	NULL	0	NULL	 plant cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review we focus our attention on cellular ROS level to trigger beneficial effects on plant cells responding to pathogen attack .
	manualset3
97666	7	400911	13	NULL	NULL	NULL	NULL	 pathogen attack	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this review we focus our attention on cellular ROS level to trigger beneficial effects on plant cells responding to pathogen attack .
	manualset3
97667	1	400912	13	NULL	NULL	0	NULL	sample	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this sample , no inpatient medical imaging examinations lengthened a stay in a way likely to be averted by digital imaging ( 95 % confidence interval 0 % to 2 % ) , and probability testing rejects the hypothesis that digital imaging will reduce hospital stays sufficiently to produce net savings at this hospital .
	manualset3
97668	2	400912	13	NULL	NULL	0	NULL	inpatient medical imaging examinations 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this sample , no inpatient medical imaging examinations lengthened a stay in a way likely to be averted by digital imaging ( 95 % confidence interval 0 % to 2 % ) , and probability testing rejects the hypothesis that digital imaging will reduce hospital stays sufficiently to produce net savings at this hospital .
	manualset3
97670	4	400912	13	NULL	NULL	0	NULL	way 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this sample , no inpatient medical imaging examinations lengthened a stay in a way likely to be averted by digital imaging ( 95 % confidence interval 0 % to 2 % ) , and probability testing rejects the hypothesis that digital imaging will reduce hospital stays sufficiently to produce net savings at this hospital .
	manualset3
97671	5	400912	13	NULL	NULL	0	NULL	digital imaging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this sample , no inpatient medical imaging examinations lengthened a stay in a way likely to be averted by digital imaging ( 95 % confidence interval 0 % to 2 % ) , and probability testing rejects the hypothesis that digital imaging will reduce hospital stays sufficiently to produce net savings at this hospital .
	manualset3
97672	6	400912	13	NULL	NULL	0	NULL	95 % confidence interval 0 % to 2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this sample , no inpatient medical imaging examinations lengthened a stay in a way likely to be averted by digital imaging ( 95 % confidence interval 0 % to 2 % ) , and probability testing rejects the hypothesis that digital imaging will reduce hospital stays sufficiently to produce net savings at this hospital .
	manualset3
97673	7	400912	13	NULL	NULL	0	NULL	probability testing 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this sample , no inpatient medical imaging examinations lengthened a stay in a way likely to be averted by digital imaging ( 95 % confidence interval 0 % to 2 % ) , and probability testing rejects the hypothesis that digital imaging will reduce hospital stays sufficiently to produce net savings at this hospital .
	manualset3
97674	8	400912	13	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this sample , no inpatient medical imaging examinations lengthened a stay in a way likely to be averted by digital imaging ( 95 % confidence interval 0 % to 2 % ) , and probability testing rejects the hypothesis that digital imaging will reduce hospital stays sufficiently to produce net savings at this hospital .
	manualset3
97675	9	400912	13	NULL	NULL	0	NULL	digital imaging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this sample , no inpatient medical imaging examinations lengthened a stay in a way likely to be averted by digital imaging ( 95 % confidence interval 0 % to 2 % ) , and probability testing rejects the hypothesis that digital imaging will reduce hospital stays sufficiently to produce net savings at this hospital .
	manualset3
97676	10	400912	13	NULL	NULL	NULL	NULL	hospital stays	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this sample , no inpatient medical imaging examinations lengthened a stay in a way likely to be averted by digital imaging ( 95 % confidence interval 0 % to 2 % ) , and probability testing rejects the hypothesis that digital imaging will reduce hospital stays sufficiently to produce net savings at this hospital .
	manualset3
97677	11	400912	13	NULL	NULL	0	NULL	net savings	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this sample , no inpatient medical imaging examinations lengthened a stay in a way likely to be averted by digital imaging ( 95 % confidence interval 0 % to 2 % ) , and probability testing rejects the hypothesis that digital imaging will reduce hospital stays sufficiently to produce net savings at this hospital .
	manualset3
97678	12	400912	13	NULL	NULL	0	NULL	hospital 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this sample , no inpatient medical imaging examinations lengthened a stay in a way likely to be averted by digital imaging ( 95 % confidence interval 0 % to 2 % ) , and probability testing rejects the hypothesis that digital imaging will reduce hospital stays sufficiently to produce net savings at this hospital .
	manualset3
97679	1	400913	13	NULL	NULL	0	NULL	 population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this selected population the most reliable diagnostic tests were CK or CK-MB isoenzymes .
	manualset3
97680	2	400913	13	NULL	NULL	0	NULL	diagnostic tests	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this selected population the most reliable diagnostic tests were CK or CK-MB isoenzymes .
	manualset3
97681	3	400913	13	NULL	NULL	0	NULL	CK isoenzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this selected population the most reliable diagnostic tests were CK or CK-MB isoenzymes .
	manualset3
97682	4	400913	13	NULL	NULL	0	NULL	CK-MB isoenzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this selected population the most reliable diagnostic tests were CK or CK-MB isoenzymes .
	manualset3
97683	1	400914	13	NULL	NULL	0	NULL	session 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In this session , Ms. Smith and Ms. Sims outlined the practice milieu for today 's nephrology nurse .
	manualset3
97684	2	400914	13	NULL	NULL	0	NULL	Ms. Smith	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In this session , Ms. Smith and Ms. Sims outlined the practice milieu for today 's nephrology nurse .
	manualset3
97685	3	400914	13	NULL	NULL	0	NULL	Ms. Sims	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In this session , Ms. Smith and Ms. Sims outlined the practice milieu for today 's nephrology nurse .
	manualset3
97686	4	400914	13	NULL	NULL	0	NULL	practice milieu	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this session , Ms. Smith and Ms. Sims outlined the practice milieu for today 's nephrology nurse .
	manualset3
97687	5	400914	13	NULL	NULL	0	NULL	nephrology nurse 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In this session , Ms. Smith and Ms. Sims outlined the practice milieu for today 's nephrology nurse .
	manualset3
97688	1	400915	13	NULL	NULL	0	NULL	communication	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this short communication , we show that in conjunction with swelling , these intuitive statements can be violated at small strains .
	manualset3
97689	2	400915	13	NULL	NULL	0	NULL	conjunction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this short communication , we show that in conjunction with swelling , these intuitive statements can be violated at small strains .
	manualset3
97690	3	400915	13	NULL	NULL	0	NULL	statements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this short communication , we show that in conjunction with swelling , these intuitive statements can be violated at small strains .
	manualset3
97691	4	400915	13	NULL	NULL	0	NULL	small strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this short communication , we show that in conjunction with swelling , these intuitive statements can be violated at small strains .
	manualset3
97692	1	400916	13	NULL	NULL	0	NULL	method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this simple and straightforward method the density of the target need not be known and only the knowledge of the target material 's mass attenuation coefficients ( composition ) for the incident and scattered energies is enough to reconstruct the density of the each voxel of the specimen being studied .
	manualset3
97693	2	400916	13	NULL	NULL	0	NULL	density of the target	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this simple and straightforward method the density of the target need not be known and only the knowledge of the target material 's mass attenuation coefficients ( composition ) for the incident and scattered energies is enough to reconstruct the density of the each voxel of the specimen being studied .
	manualset3
97694	3	400916	13	NULL	NULL	0	NULL	knowledge	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this simple and straightforward method the density of the target need not be known and only the knowledge of the target material 's mass attenuation coefficients ( composition ) for the incident and scattered energies is enough to reconstruct the density of the each voxel of the specimen being studied .
	manualset3
97695	4	400916	13	NULL	NULL	0	NULL	target material 's mass attenuation coefficients ( composition ) 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this simple and straightforward method the density of the target need not be known and only the knowledge of the target material 's mass attenuation coefficients ( composition ) for the incident and scattered energies is enough to reconstruct the density of the each voxel of the specimen being studied .
	manualset3
97696	5	400916	13	NULL	NULL	0	NULL	incident energies	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this simple and straightforward method the density of the target need not be known and only the knowledge of the target material 's mass attenuation coefficients ( composition ) for the incident and scattered energies is enough to reconstruct the density of the each voxel of the specimen being studied .
	manualset3
97697	6	400916	13	NULL	NULL	0	NULL	 scattered energies	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this simple and straightforward method the density of the target need not be known and only the knowledge of the target material 's mass attenuation coefficients ( composition ) for the incident and scattered energies is enough to reconstruct the density of the each voxel of the specimen being studied .
	manualset3
97698	7	400916	13	NULL	NULL	0	NULL	density	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this simple and straightforward method the density of the target need not be known and only the knowledge of the target material 's mass attenuation coefficients ( composition ) for the incident and scattered energies is enough to reconstruct the density of the each voxel of the specimen being studied .
	manualset3
97699	8	400916	13	NULL	NULL	0	NULL	voxel of the specimen	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this simple and straightforward method the density of the target need not be known and only the knowledge of the target material 's mass attenuation coefficients ( composition ) for the incident and scattered energies is enough to reconstruct the density of the each voxel of the specimen being studied .
	manualset3
97700	1	400917	13	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , 132 judges from three states read a murder case summary , evaluated the defendant 's guilt , assessed the voluntariness of his confession , and responded to implicit and explicit measures of harmless error .
	manualset3
97701	2	400917	13	NULL	NULL	0	NULL	132 judges 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , 132 judges from three states read a murder case summary , evaluated the defendant 's guilt , assessed the voluntariness of his confession , and responded to implicit and explicit measures of harmless error .
	manualset3
97702	3	400917	13	NULL	NULL	0	NULL	three states	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , 132 judges from three states read a murder case summary , evaluated the defendant 's guilt , assessed the voluntariness of his confession , and responded to implicit and explicit measures of harmless error .
	manualset3
97703	4	400917	13	NULL	NULL	0	NULL	 murder case summary	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , 132 judges from three states read a murder case summary , evaluated the defendant 's guilt , assessed the voluntariness of his confession , and responded to implicit and explicit measures of harmless error .
	manualset3
97704	5	400917	13	NULL	NULL	0	NULL	defendant 's	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , 132 judges from three states read a murder case summary , evaluated the defendant 's guilt , assessed the voluntariness of his confession , and responded to implicit and explicit measures of harmless error .
	manualset3
97705	6	400917	13	NULL	NULL	0	NULL	guilt	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , 132 judges from three states read a murder case summary , evaluated the defendant 's guilt , assessed the voluntariness of his confession , and responded to implicit and explicit measures of harmless error .
	manualset3
97706	7	400917	13	NULL	NULL	0	NULL	 voluntariness	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , 132 judges from three states read a murder case summary , evaluated the defendant 's guilt , assessed the voluntariness of his confession , and responded to implicit and explicit measures of harmless error .
	manualset3
97707	8	400917	13	NULL	NULL	0	NULL	 confession	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , 132 judges from three states read a murder case summary , evaluated the defendant 's guilt , assessed the voluntariness of his confession , and responded to implicit and explicit measures of harmless error .
	manualset3
97708	9	400917	13	NULL	NULL	0	NULL	 implicit measures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , 132 judges from three states read a murder case summary , evaluated the defendant 's guilt , assessed the voluntariness of his confession , and responded to implicit and explicit measures of harmless error .
	manualset3
97709	10	400917	13	NULL	NULL	0	NULL	explicit measures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , 132 judges from three states read a murder case summary , evaluated the defendant 's guilt , assessed the voluntariness of his confession , and responded to implicit and explicit measures of harmless error .
	manualset3
97710	11	400917	13	NULL	NULL	0	NULL	 error	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , 132 judges from three states read a murder case summary , evaluated the defendant 's guilt , assessed the voluntariness of his confession , and responded to implicit and explicit measures of harmless error .
	manualset3
97711	1	400918	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , Ca ( 2 + ) / CaM-dependent protein kinase ( CaMK-II ) is identified as a necessary target of this Ca ( 2 + ) elevation in zebrafish embryos .
	manualset3
97712	2	400918	13	NULL	NULL	0	NULL	Ca ( 2 + ) / CaM-dependent protein kinase ( CaMK-II )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , Ca ( 2 + ) / CaM-dependent protein kinase ( CaMK-II ) is identified as a necessary target of this Ca ( 2 + ) elevation in zebrafish embryos .
	manualset3
97713	3	400918	13	NULL	NULL	0	NULL	target	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , Ca ( 2 + ) / CaM-dependent protein kinase ( CaMK-II ) is identified as a necessary target of this Ca ( 2 + ) elevation in zebrafish embryos .
	manualset3
97714	4	400918	13	NULL	NULL	0	NULL	Ca ( 2 + ) elevation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , Ca ( 2 + ) / CaM-dependent protein kinase ( CaMK-II ) is identified as a necessary target of this Ca ( 2 + ) elevation in zebrafish embryos .
	manualset3
97715	5	400918	13	NULL	NULL	0	NULL	zebrafish embryos 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , Ca ( 2 + ) / CaM-dependent protein kinase ( CaMK-II ) is identified as a necessary target of this Ca ( 2 + ) elevation in zebrafish embryos .
	manualset3
97716	1	400919	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , FG component 1 was prepared by recycling cryoprecipitation from single-donor plasma .
	manualset3
97717	2	400919	13	NULL	NULL	0	NULL	 FG component 1	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , FG component 1 was prepared by recycling cryoprecipitation from single-donor plasma .
	manualset3
97718	3	400919	13	NULL	NULL	0	NULL	cryoprecipitation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , FG component 1 was prepared by recycling cryoprecipitation from single-donor plasma .
	manualset3
97719	4	400919	13	NULL	NULL	0	NULL	 single-donor plasma	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , FG component 1 was prepared by recycling cryoprecipitation from single-donor plasma .
	manualset3
97720	1	400920	13	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , Pseudomonas aeruginosa AA 112 which was isolated from soil using enrichment technique could utilize the malathion as a sole carbon source and a source of energy .
	manualset3
97721	2	400920	13	NULL	NULL	0	NULL	Pseudomonas aeruginosa AA 112	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , Pseudomonas aeruginosa AA 112 which was isolated from soil using enrichment technique could utilize the malathion as a sole carbon source and a source of energy .
	manualset3
97722	3	400920	13	NULL	NULL	0	NULL	soil 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , Pseudomonas aeruginosa AA 112 which was isolated from soil using enrichment technique could utilize the malathion as a sole carbon source and a source of energy .
	manualset3
97723	4	400920	13	NULL	NULL	0	NULL	enrichment technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , Pseudomonas aeruginosa AA 112 which was isolated from soil using enrichment technique could utilize the malathion as a sole carbon source and a source of energy .
	manualset3
97724	5	400920	13	NULL	NULL	0	NULL	 malathion	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , Pseudomonas aeruginosa AA 112 which was isolated from soil using enrichment technique could utilize the malathion as a sole carbon source and a source of energy .
	manualset3
97725	6	400920	13	NULL	NULL	0	NULL	carbon source	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , Pseudomonas aeruginosa AA 112 which was isolated from soil using enrichment technique could utilize the malathion as a sole carbon source and a source of energy .
	manualset3
97726	7	400920	13	NULL	NULL	0	NULL	source of energy	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , Pseudomonas aeruginosa AA 112 which was isolated from soil using enrichment technique could utilize the malathion as a sole carbon source and a source of energy .
	manualset3
97727	1	400921	13	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , a higher ADL , visiting the same dentist and cleaning teeth/dentures three or more times per day were associated with having regular dental check-ups in the elderly .
	manualset3
97728	2	400921	13	NULL	NULL	0	NULL	higher ADL	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , a higher ADL , visiting the same dentist and cleaning teeth/dentures three or more times per day were associated with having regular dental check-ups in the elderly .
	manualset3
97729	3	400921	13	NULL	NULL	0	NULL	dentist 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , a higher ADL , visiting the same dentist and cleaning teeth/dentures three or more times per day were associated with having regular dental check-ups in the elderly .
	manualset3
97730	4	400921	13	NULL	NULL	0	NULL	cleaning teeth	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , a higher ADL , visiting the same dentist and cleaning teeth/dentures three or more times per day were associated with having regular dental check-ups in the elderly .
	manualset3
97731	5	400921	13	NULL	NULL	0	NULL	dentures	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , a higher ADL , visiting the same dentist and cleaning teeth/dentures three or more times per day were associated with having regular dental check-ups in the elderly .
	manualset3
97732	6	400921	13	NULL	NULL	0	NULL	three or more times per day	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , a higher ADL , visiting the same dentist and cleaning teeth/dentures three or more times per day were associated with having regular dental check-ups in the elderly .
	manualset3
97733	7	400921	13	NULL	NULL	0	NULL	regular dental check-ups	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , a higher ADL , visiting the same dentist and cleaning teeth/dentures three or more times per day were associated with having regular dental check-ups in the elderly .
	manualset3
97734	1	400922	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , an in vivo solid phase micro-extraction ( SPME ) approach was developed and applied to the measurement of a variety of emerging contaminants ( carbamazepine , naproxen , diclofenac , gemfibrozil , bisphenol A , fluoxetine , ibuprofen and atrazine ) in fish .
	manualset3
97735	2	400922	13	NULL	NULL	0	NULL	in vivo solid phase micro-extraction ( SPME ) approach	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , an in vivo solid phase micro-extraction ( SPME ) approach was developed and applied to the measurement of a variety of emerging contaminants ( carbamazepine , naproxen , diclofenac , gemfibrozil , bisphenol A , fluoxetine , ibuprofen and atrazine ) in fish .
	manualset3
97736	3	400922	13	NULL	NULL	0	NULL	measurement	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , an in vivo solid phase micro-extraction ( SPME ) approach was developed and applied to the measurement of a variety of emerging contaminants ( carbamazepine , naproxen , diclofenac , gemfibrozil , bisphenol A , fluoxetine , ibuprofen and atrazine ) in fish .
	manualset3
97737	4	400922	13	NULL	NULL	NULL	NULL	variety of emerging contaminants 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , an in vivo solid phase micro-extraction ( SPME ) approach was developed and applied to the measurement of a variety of emerging contaminants ( carbamazepine , naproxen , diclofenac , gemfibrozil , bisphenol A , fluoxetine , ibuprofen and atrazine ) in fish .
	manualset3
97738	5	400922	13	NULL	NULL	NULL	NULL	carbamazepine 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , an in vivo solid phase micro-extraction ( SPME ) approach was developed and applied to the measurement of a variety of emerging contaminants ( carbamazepine , naproxen , diclofenac , gemfibrozil , bisphenol A , fluoxetine , ibuprofen and atrazine ) in fish .
	manualset3
97739	6	400922	13	NULL	NULL	NULL	NULL	naproxen	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , an in vivo solid phase micro-extraction ( SPME ) approach was developed and applied to the measurement of a variety of emerging contaminants ( carbamazepine , naproxen , diclofenac , gemfibrozil , bisphenol A , fluoxetine , ibuprofen and atrazine ) in fish .
	manualset3
97740	7	400922	13	NULL	NULL	NULL	NULL	diclofenac	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , an in vivo solid phase micro-extraction ( SPME ) approach was developed and applied to the measurement of a variety of emerging contaminants ( carbamazepine , naproxen , diclofenac , gemfibrozil , bisphenol A , fluoxetine , ibuprofen and atrazine ) in fish .
	manualset3
97741	8	400922	13	NULL	NULL	NULL	NULL	gemfibrozil	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , an in vivo solid phase micro-extraction ( SPME ) approach was developed and applied to the measurement of a variety of emerging contaminants ( carbamazepine , naproxen , diclofenac , gemfibrozil , bisphenol A , fluoxetine , ibuprofen and atrazine ) in fish .
	manualset3
97742	9	400922	13	NULL	NULL	NULL	NULL	bisphenol A	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , an in vivo solid phase micro-extraction ( SPME ) approach was developed and applied to the measurement of a variety of emerging contaminants ( carbamazepine , naproxen , diclofenac , gemfibrozil , bisphenol A , fluoxetine , ibuprofen and atrazine ) in fish .
	manualset3
97743	10	400922	13	NULL	NULL	NULL	NULL	fluoxetine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , an in vivo solid phase micro-extraction ( SPME ) approach was developed and applied to the measurement of a variety of emerging contaminants ( carbamazepine , naproxen , diclofenac , gemfibrozil , bisphenol A , fluoxetine , ibuprofen and atrazine ) in fish .
	manualset3
97744	11	400922	13	NULL	NULL	0	NULL	ibuprofen	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , an in vivo solid phase micro-extraction ( SPME ) approach was developed and applied to the measurement of a variety of emerging contaminants ( carbamazepine , naproxen , diclofenac , gemfibrozil , bisphenol A , fluoxetine , ibuprofen and atrazine ) in fish .
	manualset3
97745	12	400922	13	NULL	NULL	0	NULL	atrazine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , an in vivo solid phase micro-extraction ( SPME ) approach was developed and applied to the measurement of a variety of emerging contaminants ( carbamazepine , naproxen , diclofenac , gemfibrozil , bisphenol A , fluoxetine , ibuprofen and atrazine ) in fish .
	manualset3
97746	13	400922	13	NULL	NULL	0	NULL	fish	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , an in vivo solid phase micro-extraction ( SPME ) approach was developed and applied to the measurement of a variety of emerging contaminants ( carbamazepine , naproxen , diclofenac , gemfibrozil , bisphenol A , fluoxetine , ibuprofen and atrazine ) in fish .
	manualset3
97747	1	400923	13	NULL	NULL	0	NULL	Arabidopsis thaliana	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Arabidopsis thaliana ) , phospholipase D beta 1 isoform 1a ( Gossypium hirsutum ) , and PG1 ( Hordeum vulgare ) .
	manualset3
97748	2	400923	13	NULL	NULL	0	NULL	phospholipase D beta 1 isoform 1a	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Arabidopsis thaliana ) , phospholipase D beta 1 isoform 1a ( Gossypium hirsutum ) , and PG1 ( Hordeum vulgare ) .
	manualset3
97749	3	400923	13	NULL	NULL	0	NULL	Gossypium hirsutum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Arabidopsis thaliana ) , phospholipase D beta 1 isoform 1a ( Gossypium hirsutum ) , and PG1 ( Hordeum vulgare ) .
	manualset3
97750	4	400923	13	NULL	NULL	0	NULL	PG1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Arabidopsis thaliana ) , phospholipase D beta 1 isoform 1a ( Gossypium hirsutum ) , and PG1 ( Hordeum vulgare ) .
	manualset3
97751	5	400923	13	NULL	NULL	0	NULL	Hordeum vulgare 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Arabidopsis thaliana ) , phospholipase D beta 1 isoform 1a ( Gossypium hirsutum ) , and PG1 ( Hordeum vulgare ) .
	manualset3
97752	1	400924	13	NULL	NULL	0	NULL	186 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	186 patients were submitted to calcaneal ultrasound densitometry and to radiography of the dorsolumbar spine ; we also investigated the body mass index and postmenopausal and menopausal ages to identify the variable with the highest correlation with fracture , with the multiple regression statistical analysis .
	manualset3
97753	2	400924	13	NULL	NULL	0	NULL	calcaneal ultrasound densitometry	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	186 patients were submitted to calcaneal ultrasound densitometry and to radiography of the dorsolumbar spine ; we also investigated the body mass index and postmenopausal and menopausal ages to identify the variable with the highest correlation with fracture , with the multiple regression statistical analysis .
	manualset3
97754	3	400924	13	NULL	NULL	0	NULL	radiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	186 patients were submitted to calcaneal ultrasound densitometry and to radiography of the dorsolumbar spine ; we also investigated the body mass index and postmenopausal and menopausal ages to identify the variable with the highest correlation with fracture , with the multiple regression statistical analysis .
	manualset3
97755	4	400924	13	NULL	NULL	0	NULL	dorsolumbar spine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	186 patients were submitted to calcaneal ultrasound densitometry and to radiography of the dorsolumbar spine ; we also investigated the body mass index and postmenopausal and menopausal ages to identify the variable with the highest correlation with fracture , with the multiple regression statistical analysis .
	manualset3
97756	5	400924	13	NULL	NULL	0	NULL	body mass index 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	186 patients were submitted to calcaneal ultrasound densitometry and to radiography of the dorsolumbar spine ; we also investigated the body mass index and postmenopausal and menopausal ages to identify the variable with the highest correlation with fracture , with the multiple regression statistical analysis .
	manualset3
97757	6	400924	13	NULL	NULL	0	NULL	postmenopausal ages 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	186 patients were submitted to calcaneal ultrasound densitometry and to radiography of the dorsolumbar spine ; we also investigated the body mass index and postmenopausal and menopausal ages to identify the variable with the highest correlation with fracture , with the multiple regression statistical analysis .
	manualset3
97758	7	400924	13	NULL	NULL	0	NULL	menopausal ages 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	186 patients were submitted to calcaneal ultrasound densitometry and to radiography of the dorsolumbar spine ; we also investigated the body mass index and postmenopausal and menopausal ages to identify the variable with the highest correlation with fracture , with the multiple regression statistical analysis .
	manualset3
97759	8	400924	13	NULL	NULL	0	NULL	variable	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	186 patients were submitted to calcaneal ultrasound densitometry and to radiography of the dorsolumbar spine ; we also investigated the body mass index and postmenopausal and menopausal ages to identify the variable with the highest correlation with fracture , with the multiple regression statistical analysis .
	manualset3
97760	9	400924	13	NULL	NULL	0	NULL	highest correlation with fracture	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	186 patients were submitted to calcaneal ultrasound densitometry and to radiography of the dorsolumbar spine ; we also investigated the body mass index and postmenopausal and menopausal ages to identify the variable with the highest correlation with fracture , with the multiple regression statistical analysis .
	manualset3
97761	10	400924	13	NULL	NULL	0	NULL	 multiple regression statistical analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	186 patients were submitted to calcaneal ultrasound densitometry and to radiography of the dorsolumbar spine ; we also investigated the body mass index and postmenopausal and menopausal ages to identify the variable with the highest correlation with fracture , with the multiple regression statistical analysis .
	manualset3
97762	1	400925	13	NULL	NULL	0	NULL	 study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , an inhibitor of the proinflammatory enzyme , group IIA human secretory phospholipase A2 ( sPLA2-IIA ) , has been found to prevent collagen deposition as an important component of cardiovascular remodeling in a rat model of developing chronic hypertension .
	manualset3
97763	2	400925	13	NULL	NULL	0	NULL	inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , an inhibitor of the proinflammatory enzyme , group IIA human secretory phospholipase A2 ( sPLA2-IIA ) , has been found to prevent collagen deposition as an important component of cardiovascular remodeling in a rat model of developing chronic hypertension .
	manualset3
97764	3	400925	13	NULL	NULL	0	NULL	proinflammatory enzyme 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , an inhibitor of the proinflammatory enzyme , group IIA human secretory phospholipase A2 ( sPLA2-IIA ) , has been found to prevent collagen deposition as an important component of cardiovascular remodeling in a rat model of developing chronic hypertension .
	manualset3
97765	4	400925	13	NULL	NULL	0	NULL	group IIA human secretory phospholipase A2 ( sPLA2-IIA )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , an inhibitor of the proinflammatory enzyme , group IIA human secretory phospholipase A2 ( sPLA2-IIA ) , has been found to prevent collagen deposition as an important component of cardiovascular remodeling in a rat model of developing chronic hypertension .
	manualset3
97766	5	400925	13	NULL	NULL	0	NULL	collagen deposition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , an inhibitor of the proinflammatory enzyme , group IIA human secretory phospholipase A2 ( sPLA2-IIA ) , has been found to prevent collagen deposition as an important component of cardiovascular remodeling in a rat model of developing chronic hypertension .
	manualset3
97767	6	400925	13	NULL	NULL	0	NULL	component	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , an inhibitor of the proinflammatory enzyme , group IIA human secretory phospholipase A2 ( sPLA2-IIA ) , has been found to prevent collagen deposition as an important component of cardiovascular remodeling in a rat model of developing chronic hypertension .
	manualset3
97768	7	400925	13	NULL	NULL	0	NULL	cardiovascular remodeling in a rat model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , an inhibitor of the proinflammatory enzyme , group IIA human secretory phospholipase A2 ( sPLA2-IIA ) , has been found to prevent collagen deposition as an important component of cardiovascular remodeling in a rat model of developing chronic hypertension .
	manualset3
97769	8	400925	13	NULL	NULL	0	NULL	chronic hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , an inhibitor of the proinflammatory enzyme , group IIA human secretory phospholipase A2 ( sPLA2-IIA ) , has been found to prevent collagen deposition as an important component of cardiovascular remodeling in a rat model of developing chronic hypertension .
	manualset3
97770	1	400926	13	NULL	NULL	0	NULL	 study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , batch equilibrium experiments were carried out to investigate the influence of Pb ( NO ( 3 ) ) ( 2 ) on the sorption of p-nitrophenol ( PNP ) onto sediments in the presence of cationic surfactant cetylpyridinium chloride ( CPC ) .
	manualset3
97771	2	400926	13	NULL	NULL	0	NULL	batch equilibrium experiments 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , batch equilibrium experiments were carried out to investigate the influence of Pb ( NO ( 3 ) ) ( 2 ) on the sorption of p-nitrophenol ( PNP ) onto sediments in the presence of cationic surfactant cetylpyridinium chloride ( CPC ) .
	manualset3
97772	3	400926	13	NULL	NULL	0	NULL	influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , batch equilibrium experiments were carried out to investigate the influence of Pb ( NO ( 3 ) ) ( 2 ) on the sorption of p-nitrophenol ( PNP ) onto sediments in the presence of cationic surfactant cetylpyridinium chloride ( CPC ) .
	manualset3
97773	4	400926	13	NULL	NULL	0	NULL	Pb ( NO ( 3 ) ) ( 2 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , batch equilibrium experiments were carried out to investigate the influence of Pb ( NO ( 3 ) ) ( 2 ) on the sorption of p-nitrophenol ( PNP ) onto sediments in the presence of cationic surfactant cetylpyridinium chloride ( CPC ) .
	manualset3
97774	5	400926	13	NULL	NULL	0	NULL	sorption 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , batch equilibrium experiments were carried out to investigate the influence of Pb ( NO ( 3 ) ) ( 2 ) on the sorption of p-nitrophenol ( PNP ) onto sediments in the presence of cationic surfactant cetylpyridinium chloride ( CPC ) .
	manualset3
97775	6	400926	13	NULL	NULL	0	NULL	p-nitrophenol ( PNP ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , batch equilibrium experiments were carried out to investigate the influence of Pb ( NO ( 3 ) ) ( 2 ) on the sorption of p-nitrophenol ( PNP ) onto sediments in the presence of cationic surfactant cetylpyridinium chloride ( CPC ) .
	manualset3
97776	7	400926	13	NULL	NULL	0	NULL	sediments 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , batch equilibrium experiments were carried out to investigate the influence of Pb ( NO ( 3 ) ) ( 2 ) on the sorption of p-nitrophenol ( PNP ) onto sediments in the presence of cationic surfactant cetylpyridinium chloride ( CPC ) .
	manualset3
97777	8	400926	13	NULL	NULL	0	NULL	 presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , batch equilibrium experiments were carried out to investigate the influence of Pb ( NO ( 3 ) ) ( 2 ) on the sorption of p-nitrophenol ( PNP ) onto sediments in the presence of cationic surfactant cetylpyridinium chloride ( CPC ) .
	manualset3
97778	9	400926	13	NULL	NULL	0	NULL	cationic surfactant cetylpyridinium chloride ( CPC ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , batch equilibrium experiments were carried out to investigate the influence of Pb ( NO ( 3 ) ) ( 2 ) on the sorption of p-nitrophenol ( PNP ) onto sediments in the presence of cationic surfactant cetylpyridinium chloride ( CPC ) .
	manualset3
97779	1	400927	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , by mutating the putative WC-1 flavin-binding sites , we show that these sites are important for the light function of the protein , suggesting that the WC-1 LOV domain adapts a structure similar to that of the phototropin LOV domains .
	manualset3
97780	2	400927	13	NULL	NULL	0	NULL	putative WC-1 flavin-binding sites 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , by mutating the putative WC-1 flavin-binding sites , we show that these sites are important for the light function of the protein , suggesting that the WC-1 LOV domain adapts a structure similar to that of the phototropin LOV domains .
	manualset3
97781	3	400927	13	NULL	NULL	0	NULL	sites 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , by mutating the putative WC-1 flavin-binding sites , we show that these sites are important for the light function of the protein , suggesting that the WC-1 LOV domain adapts a structure similar to that of the phototropin LOV domains .
	manualset3
97782	4	400927	13	NULL	NULL	0	NULL	light function 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , by mutating the putative WC-1 flavin-binding sites , we show that these sites are important for the light function of the protein , suggesting that the WC-1 LOV domain adapts a structure similar to that of the phototropin LOV domains .
	manualset3
97783	5	400927	13	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , by mutating the putative WC-1 flavin-binding sites , we show that these sites are important for the light function of the protein , suggesting that the WC-1 LOV domain adapts a structure similar to that of the phototropin LOV domains .
	manualset3
97784	6	400927	13	NULL	NULL	0	NULL	WC-1 LOV domain 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , by mutating the putative WC-1 flavin-binding sites , we show that these sites are important for the light function of the protein , suggesting that the WC-1 LOV domain adapts a structure similar to that of the phototropin LOV domains .
	manualset3
97785	7	400927	13	NULL	NULL	0	NULL	structure 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , by mutating the putative WC-1 flavin-binding sites , we show that these sites are important for the light function of the protein , suggesting that the WC-1 LOV domain adapts a structure similar to that of the phototropin LOV domains .
	manualset3
97786	8	400927	13	NULL	NULL	0	NULL	phototropin LOV domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , by mutating the putative WC-1 flavin-binding sites , we show that these sites are important for the light function of the protein , suggesting that the WC-1 LOV domain adapts a structure similar to that of the phototropin LOV domains .
	manualset3
97787	1	400928	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , chickens and swine were evaluated for susceptibility to vacuolar myelinopathy with the intent of developing animal models for research and to identify specific tissues in affected coots that contain the causative agent .
	manualset3
97788	2	400928	13	NULL	NULL	0	NULL	chickens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , chickens and swine were evaluated for susceptibility to vacuolar myelinopathy with the intent of developing animal models for research and to identify specific tissues in affected coots that contain the causative agent .
	manualset3
97789	3	400928	13	NULL	NULL	0	NULL	swine	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , chickens and swine were evaluated for susceptibility to vacuolar myelinopathy with the intent of developing animal models for research and to identify specific tissues in affected coots that contain the causative agent .
	manualset3
97790	4	400928	13	NULL	NULL	0	NULL	susceptibility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , chickens and swine were evaluated for susceptibility to vacuolar myelinopathy with the intent of developing animal models for research and to identify specific tissues in affected coots that contain the causative agent .
	manualset3
97791	5	400928	13	NULL	NULL	0	NULL	vacuolar myelinopathy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , chickens and swine were evaluated for susceptibility to vacuolar myelinopathy with the intent of developing animal models for research and to identify specific tissues in affected coots that contain the causative agent .
	manualset3
97792	6	400928	13	NULL	NULL	NULL	NULL	intent	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , chickens and swine were evaluated for susceptibility to vacuolar myelinopathy with the intent of developing animal models for research and to identify specific tissues in affected coots that contain the causative agent .
	manualset3
97793	7	400928	13	NULL	NULL	0	NULL	animal models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , chickens and swine were evaluated for susceptibility to vacuolar myelinopathy with the intent of developing animal models for research and to identify specific tissues in affected coots that contain the causative agent .
	manualset3
97794	8	400928	13	NULL	NULL	0	NULL	research 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , chickens and swine were evaluated for susceptibility to vacuolar myelinopathy with the intent of developing animal models for research and to identify specific tissues in affected coots that contain the causative agent .
	manualset3
97795	9	400928	13	NULL	NULL	0	NULL	specific tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , chickens and swine were evaluated for susceptibility to vacuolar myelinopathy with the intent of developing animal models for research and to identify specific tissues in affected coots that contain the causative agent .
	manualset3
97796	10	400928	13	NULL	NULL	0	NULL	coots 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , chickens and swine were evaluated for susceptibility to vacuolar myelinopathy with the intent of developing animal models for research and to identify specific tissues in affected coots that contain the causative agent .
	manualset3
97797	11	400928	13	NULL	NULL	0	NULL	causative agent 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , chickens and swine were evaluated for susceptibility to vacuolar myelinopathy with the intent of developing animal models for research and to identify specific tissues in affected coots that contain the causative agent .
	manualset3
97798	1	400929	13	NULL	NULL	0	NULL	 study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , chondrocytes were derived from the cartilages of knee joints of 4-week-old male Sprague-Dawley rats and were mechanically digested by collagenase type II treatment for further culture in vitro .
	manualset3
97799	2	400929	13	NULL	NULL	0	NULL	 chondrocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , chondrocytes were derived from the cartilages of knee joints of 4-week-old male Sprague-Dawley rats and were mechanically digested by collagenase type II treatment for further culture in vitro .
	manualset3
97800	3	400929	13	NULL	NULL	0	NULL	cartilages of knee joints 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , chondrocytes were derived from the cartilages of knee joints of 4-week-old male Sprague-Dawley rats and were mechanically digested by collagenase type II treatment for further culture in vitro .
	manualset3
97801	4	400929	13	NULL	NULL	0	NULL	4-week-old male Sprague-Dawley rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , chondrocytes were derived from the cartilages of knee joints of 4-week-old male Sprague-Dawley rats and were mechanically digested by collagenase type II treatment for further culture in vitro .
	manualset3
97802	5	400929	13	NULL	NULL	0	NULL	collagenase type II 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , chondrocytes were derived from the cartilages of knee joints of 4-week-old male Sprague-Dawley rats and were mechanically digested by collagenase type II treatment for further culture in vitro .
	manualset3
97803	6	400929	13	NULL	NULL	0	NULL	treatment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , chondrocytes were derived from the cartilages of knee joints of 4-week-old male Sprague-Dawley rats and were mechanically digested by collagenase type II treatment for further culture in vitro .
	manualset3
97804	7	400929	13	NULL	NULL	0	NULL	culture in vitro	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , chondrocytes were derived from the cartilages of knee joints of 4-week-old male Sprague-Dawley rats and were mechanically digested by collagenase type II treatment for further culture in vitro .
	manualset3
97805	1	400930	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , data collected during PS field campaigns ( from 2004 to 2006 ) , using horizontal and differently inclined dosimeters , were analyzed to provide some considerations on the transfer of the horizontal calibration to differently inclined dosimeters , as anatomic sites usually are .
	manualset3
97806	2	400930	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , data collected during PS field campaigns ( from 2004 to 2006 ) , using horizontal and differently inclined dosimeters , were analyzed to provide some considerations on the transfer of the horizontal calibration to differently inclined dosimeters , as anatomic sites usually are .
	manualset3
97807	3	400930	13	NULL	NULL	0	NULL	PS field campaigns	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , data collected during PS field campaigns ( from 2004 to 2006 ) , using horizontal and differently inclined dosimeters , were analyzed to provide some considerations on the transfer of the horizontal calibration to differently inclined dosimeters , as anatomic sites usually are .
	manualset3
97808	4	400930	13	NULL	NULL	0	NULL	from 2004 to 2006 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , data collected during PS field campaigns ( from 2004 to 2006 ) , using horizontal and differently inclined dosimeters , were analyzed to provide some considerations on the transfer of the horizontal calibration to differently inclined dosimeters , as anatomic sites usually are .
	manualset3
97809	5	400930	13	NULL	NULL	0	NULL	 dosimeters	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , data collected during PS field campaigns ( from 2004 to 2006 ) , using horizontal and differently inclined dosimeters , were analyzed to provide some considerations on the transfer of the horizontal calibration to differently inclined dosimeters , as anatomic sites usually are .
	manualset3
97810	6	400930	13	NULL	NULL	0	NULL	considerations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , data collected during PS field campaigns ( from 2004 to 2006 ) , using horizontal and differently inclined dosimeters , were analyzed to provide some considerations on the transfer of the horizontal calibration to differently inclined dosimeters , as anatomic sites usually are .
	manualset3
97811	7	400930	13	NULL	NULL	0	NULL	 transfer 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , data collected during PS field campaigns ( from 2004 to 2006 ) , using horizontal and differently inclined dosimeters , were analyzed to provide some considerations on the transfer of the horizontal calibration to differently inclined dosimeters , as anatomic sites usually are .
	manualset3
97812	8	400930	13	NULL	NULL	0	NULL	calibration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , data collected during PS field campaigns ( from 2004 to 2006 ) , using horizontal and differently inclined dosimeters , were analyzed to provide some considerations on the transfer of the horizontal calibration to differently inclined dosimeters , as anatomic sites usually are .
	manualset3
97813	9	400930	13	NULL	NULL	0	NULL	dosimeters	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , data collected during PS field campaigns ( from 2004 to 2006 ) , using horizontal and differently inclined dosimeters , were analyzed to provide some considerations on the transfer of the horizontal calibration to differently inclined dosimeters , as anatomic sites usually are .
	manualset3
97814	10	400930	13	NULL	NULL	0	NULL	anatomic sites	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , data collected during PS field campaigns ( from 2004 to 2006 ) , using horizontal and differently inclined dosimeters , were analyzed to provide some considerations on the transfer of the horizontal calibration to differently inclined dosimeters , as anatomic sites usually are .
	manualset3
97815	1	400931	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , disease progression was defined as invasion to the muscle or further ( upstage ) and presence of metastasis ( metastasis ) .
	manualset3
97816	2	400931	13	NULL	NULL	0	NULL	disease progression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , disease progression was defined as invasion to the muscle or further ( upstage ) and presence of metastasis ( metastasis ) .
	manualset3
97817	3	400931	13	NULL	NULL	0	NULL	invasion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , disease progression was defined as invasion to the muscle or further ( upstage ) and presence of metastasis ( metastasis ) .
	manualset3
97818	4	400931	13	NULL	NULL	0	NULL	muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , disease progression was defined as invasion to the muscle or further ( upstage ) and presence of metastasis ( metastasis ) .
	manualset3
97819	5	400931	13	NULL	NULL	0	NULL	upstage	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , disease progression was defined as invasion to the muscle or further ( upstage ) and presence of metastasis ( metastasis ) .
	manualset3
97820	6	400931	13	NULL	NULL	0	NULL	 presence of metastasis ( metastasis ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , disease progression was defined as invasion to the muscle or further ( upstage ) and presence of metastasis ( metastasis ) .
	manualset3
97821	1	400932	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , our LVAS was implanted between the left atrium and the aorta in twelve goats in which the hearts were fibrillated .
	manualset3
97822	2	400932	13	NULL	NULL	0	NULL	LVAS 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , our LVAS was implanted between the left atrium and the aorta in twelve goats in which the hearts were fibrillated .
	manualset3
97823	3	400932	13	NULL	NULL	0	NULL	left atrium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , our LVAS was implanted between the left atrium and the aorta in twelve goats in which the hearts were fibrillated .
	manualset3
97824	4	400932	13	NULL	NULL	0	NULL	aorta	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , our LVAS was implanted between the left atrium and the aorta in twelve goats in which the hearts were fibrillated .
	manualset3
97825	5	400932	13	NULL	NULL	0	NULL	twelve	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , our LVAS was implanted between the left atrium and the aorta in twelve goats in which the hearts were fibrillated .
	manualset3
97826	6	400932	13	NULL	NULL	0	NULL	goats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , our LVAS was implanted between the left atrium and the aorta in twelve goats in which the hearts were fibrillated .
	manualset3
97827	7	400932	13	NULL	NULL	0	NULL	hearts 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , our LVAS was implanted between the left atrium and the aorta in twelve goats in which the hearts were fibrillated .
	manualset3
97828	1	400933	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , our intent is to describe the experiences of the authors with the treatment of rectal prolapse , to estimate the actual level of expertise of the surgeons in treatment of rectal prolapse , and to describe in which way to proceed in the future ( Tab .
	manualset3
97829	2	400933	13	NULL	NULL	0	NULL	intent	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , our intent is to describe the experiences of the authors with the treatment of rectal prolapse , to estimate the actual level of expertise of the surgeons in treatment of rectal prolapse , and to describe in which way to proceed in the future ( Tab .
	manualset3
97830	3	400933	13	NULL	NULL	0	NULL	experiences	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , our intent is to describe the experiences of the authors with the treatment of rectal prolapse , to estimate the actual level of expertise of the surgeons in treatment of rectal prolapse , and to describe in which way to proceed in the future ( Tab .
	manualset3
97831	4	400933	13	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , our intent is to describe the experiences of the authors with the treatment of rectal prolapse , to estimate the actual level of expertise of the surgeons in treatment of rectal prolapse , and to describe in which way to proceed in the future ( Tab .
	manualset3
97832	5	400933	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , our intent is to describe the experiences of the authors with the treatment of rectal prolapse , to estimate the actual level of expertise of the surgeons in treatment of rectal prolapse , and to describe in which way to proceed in the future ( Tab .
	manualset3
97833	6	400933	13	NULL	NULL	0	NULL	rectal prolapse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , our intent is to describe the experiences of the authors with the treatment of rectal prolapse , to estimate the actual level of expertise of the surgeons in treatment of rectal prolapse , and to describe in which way to proceed in the future ( Tab .
	manualset3
97834	7	400933	13	NULL	NULL	NULL	NULL	actual level of expertise 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , our intent is to describe the experiences of the authors with the treatment of rectal prolapse , to estimate the actual level of expertise of the surgeons in treatment of rectal prolapse , and to describe in which way to proceed in the future ( Tab .
	manualset3
97835	8	400933	13	NULL	NULL	0	NULL	surgeons	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , our intent is to describe the experiences of the authors with the treatment of rectal prolapse , to estimate the actual level of expertise of the surgeons in treatment of rectal prolapse , and to describe in which way to proceed in the future ( Tab .
	manualset3
97836	9	400933	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , our intent is to describe the experiences of the authors with the treatment of rectal prolapse , to estimate the actual level of expertise of the surgeons in treatment of rectal prolapse , and to describe in which way to proceed in the future ( Tab .
	manualset3
97837	10	400933	13	NULL	NULL	0	NULL	rectal prolapse 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , our intent is to describe the experiences of the authors with the treatment of rectal prolapse , to estimate the actual level of expertise of the surgeons in treatment of rectal prolapse , and to describe in which way to proceed in the future ( Tab .
	manualset3
97838	11	400933	13	NULL	NULL	NULL	NULL	way 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , our intent is to describe the experiences of the authors with the treatment of rectal prolapse , to estimate the actual level of expertise of the surgeons in treatment of rectal prolapse , and to describe in which way to proceed in the future ( Tab .
	manualset3
97839	12	400933	13	NULL	NULL	0	NULL	future	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , our intent is to describe the experiences of the authors with the treatment of rectal prolapse , to estimate the actual level of expertise of the surgeons in treatment of rectal prolapse , and to describe in which way to proceed in the future ( Tab .
	manualset3
97840	1	400934	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , plasma glucose was converted into CO ( 2 ) by an in-tube reaction with yeast permitting direct measurement of ( 13 ) CO ( 2 ) in the headspace .
	manualset3
97841	2	400934	13	NULL	NULL	0	NULL	plasma glucose	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , plasma glucose was converted into CO ( 2 ) by an in-tube reaction with yeast permitting direct measurement of ( 13 ) CO ( 2 ) in the headspace .
	manualset3
97842	3	400934	13	NULL	NULL	0	NULL	CO ( 2 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , plasma glucose was converted into CO ( 2 ) by an in-tube reaction with yeast permitting direct measurement of ( 13 ) CO ( 2 ) in the headspace .
	manualset3
97843	4	400934	13	NULL	NULL	0	NULL	in-tube reaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , plasma glucose was converted into CO ( 2 ) by an in-tube reaction with yeast permitting direct measurement of ( 13 ) CO ( 2 ) in the headspace .
	manualset3
97844	5	400934	13	NULL	NULL	0	NULL	 yeast	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , plasma glucose was converted into CO ( 2 ) by an in-tube reaction with yeast permitting direct measurement of ( 13 ) CO ( 2 ) in the headspace .
	manualset3
97845	6	400934	13	NULL	NULL	0	NULL	measurement 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , plasma glucose was converted into CO ( 2 ) by an in-tube reaction with yeast permitting direct measurement of ( 13 ) CO ( 2 ) in the headspace .
	manualset3
97846	7	400934	13	NULL	NULL	0	NULL	( 13 ) CO ( 2 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , plasma glucose was converted into CO ( 2 ) by an in-tube reaction with yeast permitting direct measurement of ( 13 ) CO ( 2 ) in the headspace .
	manualset3
97847	8	400934	13	NULL	NULL	0	NULL	headspace	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , plasma glucose was converted into CO ( 2 ) by an in-tube reaction with yeast permitting direct measurement of ( 13 ) CO ( 2 ) in the headspace .
	manualset3
97848	1	400935	13	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , sleep timing was compared between married Japanese couples ( n = 225 ) who had lived together for 1 yr or more ( mean 17 yrs ) .
	manualset3
97849	2	400935	13	NULL	NULL	0	NULL	sleep timing 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , sleep timing was compared between married Japanese couples ( n = 225 ) who had lived together for 1 yr or more ( mean 17 yrs ) .
	manualset3
97850	3	400935	13	NULL	NULL	0	NULL	Japanese couples	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , sleep timing was compared between married Japanese couples ( n = 225 ) who had lived together for 1 yr or more ( mean 17 yrs ) .
	manualset3
97851	4	400935	13	NULL	NULL	0	NULL	 n = 225	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , sleep timing was compared between married Japanese couples ( n = 225 ) who had lived together for 1 yr or more ( mean 17 yrs ) .
	manualset3
97852	5	400935	13	NULL	NULL	0	NULL	1 yr or more ( mean 17 yrs )	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , sleep timing was compared between married Japanese couples ( n = 225 ) who had lived together for 1 yr or more ( mean 17 yrs ) .
	manualset3
97853	1	400936	13	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the authors have as a goal to discuss the care-investigation interface in the caring practice of Nursing in the hospital ambit , starting from their professional experiences .
	manualset3
97854	2	400936	13	NULL	NULL	0	NULL	 authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the authors have as a goal to discuss the care-investigation interface in the caring practice of Nursing in the hospital ambit , starting from their professional experiences .
	manualset3
97855	3	400936	13	NULL	NULL	0	NULL	 goal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the authors have as a goal to discuss the care-investigation interface in the caring practice of Nursing in the hospital ambit , starting from their professional experiences .
	manualset3
97856	4	400936	13	NULL	NULL	0	NULL	care-investigation interface	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the authors have as a goal to discuss the care-investigation interface in the caring practice of Nursing in the hospital ambit , starting from their professional experiences .
	manualset3
97857	5	400936	13	NULL	NULL	NULL	NULL	practice of Nursing	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , the authors have as a goal to discuss the care-investigation interface in the caring practice of Nursing in the hospital ambit , starting from their professional experiences .
	manualset3
97858	6	400936	13	NULL	NULL	0	NULL	hospital ambit	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the authors have as a goal to discuss the care-investigation interface in the caring practice of Nursing in the hospital ambit , starting from their professional experiences .
	manualset3
97859	7	400936	13	NULL	NULL	0	NULL	professional experiences	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the authors have as a goal to discuss the care-investigation interface in the caring practice of Nursing in the hospital ambit , starting from their professional experiences .
	manualset3
97860	1	400937	13	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the authors report that sodium citrate can aggregate hexadecyl-trimethyl-ammonium ion ( + ) - coated gold nanorods ( AuNRs ) , and nucleic acids of different charge and structure properties , i.e. , single-stranded DNA ( ssDNA ) , double-stranded DNA ( dsDNA ) , single-stranded peptide nucleic acid ( PNA ) , and PNA-DNA complex , can bind to the AuNRs and therefore retard the sodium citrate-induced aggregation to different extents .
	manualset3
97861	2	400937	13	NULL	NULL	0	NULL	 authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the authors report that sodium citrate can aggregate hexadecyl-trimethyl-ammonium ion ( + ) - coated gold nanorods ( AuNRs ) , and nucleic acids of different charge and structure properties , i.e. , single-stranded DNA ( ssDNA ) , double-stranded DNA ( dsDNA ) , single-stranded peptide nucleic acid ( PNA ) , and PNA-DNA complex , can bind to the AuNRs and therefore retard the sodium citrate-induced aggregation to different extents .
	manualset3
97862	3	400937	13	NULL	NULL	0	NULL	sodium citrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the authors report that sodium citrate can aggregate hexadecyl-trimethyl-ammonium ion ( + ) - coated gold nanorods ( AuNRs ) , and nucleic acids of different charge and structure properties , i.e. , single-stranded DNA ( ssDNA ) , double-stranded DNA ( dsDNA ) , single-stranded peptide nucleic acid ( PNA ) , and PNA-DNA complex , can bind to the AuNRs and therefore retard the sodium citrate-induced aggregation to different extents .
	manualset3
97863	4	400937	13	NULL	NULL	0	NULL	 hexadecyl-trimethyl-ammonium ion ( + ) - coated gold nanorods ( AuNRs ) 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the authors report that sodium citrate can aggregate hexadecyl-trimethyl-ammonium ion ( + ) - coated gold nanorods ( AuNRs ) , and nucleic acids of different charge and structure properties , i.e. , single-stranded DNA ( ssDNA ) , double-stranded DNA ( dsDNA ) , single-stranded peptide nucleic acid ( PNA ) , and PNA-DNA complex , can bind to the AuNRs and therefore retard the sodium citrate-induced aggregation to different extents .
	manualset3
97864	5	400937	13	NULL	NULL	0	NULL	nucleic acids of different charge	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the authors report that sodium citrate can aggregate hexadecyl-trimethyl-ammonium ion ( + ) - coated gold nanorods ( AuNRs ) , and nucleic acids of different charge and structure properties , i.e. , single-stranded DNA ( ssDNA ) , double-stranded DNA ( dsDNA ) , single-stranded peptide nucleic acid ( PNA ) , and PNA-DNA complex , can bind to the AuNRs and therefore retard the sodium citrate-induced aggregation to different extents .
	manualset3
97865	6	400937	13	NULL	NULL	0	NULL	structure properties	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the authors report that sodium citrate can aggregate hexadecyl-trimethyl-ammonium ion ( + ) - coated gold nanorods ( AuNRs ) , and nucleic acids of different charge and structure properties , i.e. , single-stranded DNA ( ssDNA ) , double-stranded DNA ( dsDNA ) , single-stranded peptide nucleic acid ( PNA ) , and PNA-DNA complex , can bind to the AuNRs and therefore retard the sodium citrate-induced aggregation to different extents .
	manualset3
97866	7	400937	13	NULL	NULL	0	NULL	single-stranded DNA ( ssDNA ) 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the authors report that sodium citrate can aggregate hexadecyl-trimethyl-ammonium ion ( + ) - coated gold nanorods ( AuNRs ) , and nucleic acids of different charge and structure properties , i.e. , single-stranded DNA ( ssDNA ) , double-stranded DNA ( dsDNA ) , single-stranded peptide nucleic acid ( PNA ) , and PNA-DNA complex , can bind to the AuNRs and therefore retard the sodium citrate-induced aggregation to different extents .
	manualset3
97867	8	400937	13	NULL	NULL	0	NULL	 double-stranded DNA ( dsDNA )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the authors report that sodium citrate can aggregate hexadecyl-trimethyl-ammonium ion ( + ) - coated gold nanorods ( AuNRs ) , and nucleic acids of different charge and structure properties , i.e. , single-stranded DNA ( ssDNA ) , double-stranded DNA ( dsDNA ) , single-stranded peptide nucleic acid ( PNA ) , and PNA-DNA complex , can bind to the AuNRs and therefore retard the sodium citrate-induced aggregation to different extents .
	manualset3
97868	9	400937	13	NULL	NULL	0	NULL	single-stranded peptide nucleic acid ( PNA )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the authors report that sodium citrate can aggregate hexadecyl-trimethyl-ammonium ion ( + ) - coated gold nanorods ( AuNRs ) , and nucleic acids of different charge and structure properties , i.e. , single-stranded DNA ( ssDNA ) , double-stranded DNA ( dsDNA ) , single-stranded peptide nucleic acid ( PNA ) , and PNA-DNA complex , can bind to the AuNRs and therefore retard the sodium citrate-induced aggregation to different extents .
	manualset3
97869	10	400937	13	NULL	NULL	0	NULL	PNA-DNA complex 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the authors report that sodium citrate can aggregate hexadecyl-trimethyl-ammonium ion ( + ) - coated gold nanorods ( AuNRs ) , and nucleic acids of different charge and structure properties , i.e. , single-stranded DNA ( ssDNA ) , double-stranded DNA ( dsDNA ) , single-stranded peptide nucleic acid ( PNA ) , and PNA-DNA complex , can bind to the AuNRs and therefore retard the sodium citrate-induced aggregation to different extents .
	manualset3
97870	11	400937	13	NULL	NULL	0	NULL	AuNRs	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the authors report that sodium citrate can aggregate hexadecyl-trimethyl-ammonium ion ( + ) - coated gold nanorods ( AuNRs ) , and nucleic acids of different charge and structure properties , i.e. , single-stranded DNA ( ssDNA ) , double-stranded DNA ( dsDNA ) , single-stranded peptide nucleic acid ( PNA ) , and PNA-DNA complex , can bind to the AuNRs and therefore retard the sodium citrate-induced aggregation to different extents .
	manualset3
97871	12	400937	13	NULL	NULL	0	NULL	 sodium citrate-induced aggregation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the authors report that sodium citrate can aggregate hexadecyl-trimethyl-ammonium ion ( + ) - coated gold nanorods ( AuNRs ) , and nucleic acids of different charge and structure properties , i.e. , single-stranded DNA ( ssDNA ) , double-stranded DNA ( dsDNA ) , single-stranded peptide nucleic acid ( PNA ) , and PNA-DNA complex , can bind to the AuNRs and therefore retard the sodium citrate-induced aggregation to different extents .
	manualset3
97872	13	400937	13	NULL	NULL	0	NULL	different extents	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the authors report that sodium citrate can aggregate hexadecyl-trimethyl-ammonium ion ( + ) - coated gold nanorods ( AuNRs ) , and nucleic acids of different charge and structure properties , i.e. , single-stranded DNA ( ssDNA ) , double-stranded DNA ( dsDNA ) , single-stranded peptide nucleic acid ( PNA ) , and PNA-DNA complex , can bind to the AuNRs and therefore retard the sodium citrate-induced aggregation to different extents .
	manualset3
97873	1	400938	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the efficacy of SCG could not be related to age , atopic status , the initial level of allergen-specific IgE antibody , baseline FEV1 , level of bronchial responsiveness to inhaled histamine or an effect of SCG on responsiveness to histamine .
	manualset3
97874	2	400938	13	NULL	NULL	0	NULL	efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the efficacy of SCG could not be related to age , atopic status , the initial level of allergen-specific IgE antibody , baseline FEV1 , level of bronchial responsiveness to inhaled histamine or an effect of SCG on responsiveness to histamine .
	manualset3
97875	3	400938	13	NULL	NULL	0	NULL	SCG 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the efficacy of SCG could not be related to age , atopic status , the initial level of allergen-specific IgE antibody , baseline FEV1 , level of bronchial responsiveness to inhaled histamine or an effect of SCG on responsiveness to histamine .
	manualset3
97876	4	400938	13	NULL	NULL	0	NULL	age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the efficacy of SCG could not be related to age , atopic status , the initial level of allergen-specific IgE antibody , baseline FEV1 , level of bronchial responsiveness to inhaled histamine or an effect of SCG on responsiveness to histamine .
	manualset3
97877	5	400938	13	NULL	NULL	0	NULL	atopic status 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the efficacy of SCG could not be related to age , atopic status , the initial level of allergen-specific IgE antibody , baseline FEV1 , level of bronchial responsiveness to inhaled histamine or an effect of SCG on responsiveness to histamine .
	manualset3
97878	6	400938	13	NULL	NULL	NULL	NULL	 initial level of allergen-specific IgE antibody	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , the efficacy of SCG could not be related to age , atopic status , the initial level of allergen-specific IgE antibody , baseline FEV1 , level of bronchial responsiveness to inhaled histamine or an effect of SCG on responsiveness to histamine .
	manualset3
97879	7	400938	13	NULL	NULL	0	NULL	baseline FEV1 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the efficacy of SCG could not be related to age , atopic status , the initial level of allergen-specific IgE antibody , baseline FEV1 , level of bronchial responsiveness to inhaled histamine or an effect of SCG on responsiveness to histamine .
	manualset3
97880	8	400938	13	NULL	NULL	0	NULL	level of bronchial responsiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the efficacy of SCG could not be related to age , atopic status , the initial level of allergen-specific IgE antibody , baseline FEV1 , level of bronchial responsiveness to inhaled histamine or an effect of SCG on responsiveness to histamine .
	manualset3
97881	9	400938	13	NULL	NULL	0	NULL	histamine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the efficacy of SCG could not be related to age , atopic status , the initial level of allergen-specific IgE antibody , baseline FEV1 , level of bronchial responsiveness to inhaled histamine or an effect of SCG on responsiveness to histamine .
	manualset3
97882	10	400938	13	NULL	NULL	0	NULL	effect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the efficacy of SCG could not be related to age , atopic status , the initial level of allergen-specific IgE antibody , baseline FEV1 , level of bronchial responsiveness to inhaled histamine or an effect of SCG on responsiveness to histamine .
	manualset3
97883	11	400938	13	NULL	NULL	0	NULL	SCG	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the efficacy of SCG could not be related to age , atopic status , the initial level of allergen-specific IgE antibody , baseline FEV1 , level of bronchial responsiveness to inhaled histamine or an effect of SCG on responsiveness to histamine .
	manualset3
97884	12	400938	13	NULL	NULL	0	NULL	responsiveness to histamine	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the efficacy of SCG could not be related to age , atopic status , the initial level of allergen-specific IgE antibody , baseline FEV1 , level of bronchial responsiveness to inhaled histamine or an effect of SCG on responsiveness to histamine .
	manualset3
97885	1	400939	13	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the efficacy of a commercially produced type III secreted protein ( TTSP ) vaccine was evaluated with the use of a commingled experimental calf infection model ( 30 placebo-treated animals and 30 vaccinates ) .
	manualset3
97886	2	400939	13	NULL	NULL	0	NULL	 efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the efficacy of a commercially produced type III secreted protein ( TTSP ) vaccine was evaluated with the use of a commingled experimental calf infection model ( 30 placebo-treated animals and 30 vaccinates ) .
	manualset3
97887	3	400939	13	NULL	NULL	0	NULL	type III secreted protein ( TTSP ) vaccine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the efficacy of a commercially produced type III secreted protein ( TTSP ) vaccine was evaluated with the use of a commingled experimental calf infection model ( 30 placebo-treated animals and 30 vaccinates ) .
	manualset3
97888	4	400939	13	NULL	NULL	0	NULL	use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the efficacy of a commercially produced type III secreted protein ( TTSP ) vaccine was evaluated with the use of a commingled experimental calf infection model ( 30 placebo-treated animals and 30 vaccinates ) .
	manualset3
97889	5	400939	13	NULL	NULL	0	NULL	experimental calf infection model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the efficacy of a commercially produced type III secreted protein ( TTSP ) vaccine was evaluated with the use of a commingled experimental calf infection model ( 30 placebo-treated animals and 30 vaccinates ) .
	manualset3
97890	6	400939	13	NULL	NULL	0	NULL	30 placebo-treated animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the efficacy of a commercially produced type III secreted protein ( TTSP ) vaccine was evaluated with the use of a commingled experimental calf infection model ( 30 placebo-treated animals and 30 vaccinates ) .
	manualset3
97891	7	400939	13	NULL	NULL	0	NULL	30 vaccinates 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the efficacy of a commercially produced type III secreted protein ( TTSP ) vaccine was evaluated with the use of a commingled experimental calf infection model ( 30 placebo-treated animals and 30 vaccinates ) .
	manualset3
97892	1	400940	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the full ejection trigger level for the current beat was changed based on the estimated afterload derived from the previous beat 's pressure waveform .
	manualset3
97893	2	400940	13	NULL	NULL	0	NULL	full ejection trigger level	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the full ejection trigger level for the current beat was changed based on the estimated afterload derived from the previous beat 's pressure waveform .
	manualset3
97894	3	400940	13	NULL	NULL	0	NULL	beat	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the full ejection trigger level for the current beat was changed based on the estimated afterload derived from the previous beat 's pressure waveform .
	manualset3
97895	4	400940	13	NULL	NULL	0	NULL	afterload 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the full ejection trigger level for the current beat was changed based on the estimated afterload derived from the previous beat 's pressure waveform .
	manualset3
97896	5	400940	13	NULL	NULL	0	NULL	beat 's pressure waveform 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the full ejection trigger level for the current beat was changed based on the estimated afterload derived from the previous beat 's pressure waveform .
	manualset3
97897	1	400941	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the functional contributions of Ca ( 2 + ) transporters to ( Ca ( 2 + ) ) ( i ) decline in mouse embryonic stem cell-derived cardiomyocytes ( mESCMs ) , a suitable model for investigation of early cardiogenesis , at various differentiation stages were investigated .
	manualset3
97898	2	400941	13	NULL	NULL	0	NULL	functional contributions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the functional contributions of Ca ( 2 + ) transporters to ( Ca ( 2 + ) ) ( i ) decline in mouse embryonic stem cell-derived cardiomyocytes ( mESCMs ) , a suitable model for investigation of early cardiogenesis , at various differentiation stages were investigated .
	manualset3
97899	3	400941	13	NULL	NULL	0	NULL	 Ca ( 2 + ) transporters 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the functional contributions of Ca ( 2 + ) transporters to ( Ca ( 2 + ) ) ( i ) decline in mouse embryonic stem cell-derived cardiomyocytes ( mESCMs ) , a suitable model for investigation of early cardiogenesis , at various differentiation stages were investigated .
	manualset3
97900	4	400941	13	NULL	NULL	0	NULL	Ca ( 2 + ) 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the functional contributions of Ca ( 2 + ) transporters to ( Ca ( 2 + ) ) ( i ) decline in mouse embryonic stem cell-derived cardiomyocytes ( mESCMs ) , a suitable model for investigation of early cardiogenesis , at various differentiation stages were investigated .
	manualset3
97902	6	400941	13	NULL	NULL	0	NULL	mouse embryonic stem cell-derived cardiomyocytes ( mESCMs )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the functional contributions of Ca ( 2 + ) transporters to ( Ca ( 2 + ) ) ( i ) decline in mouse embryonic stem cell-derived cardiomyocytes ( mESCMs ) , a suitable model for investigation of early cardiogenesis , at various differentiation stages were investigated .
	manualset3
97903	7	400941	13	NULL	NULL	0	NULL	model for investigation 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the functional contributions of Ca ( 2 + ) transporters to ( Ca ( 2 + ) ) ( i ) decline in mouse embryonic stem cell-derived cardiomyocytes ( mESCMs ) , a suitable model for investigation of early cardiogenesis , at various differentiation stages were investigated .
	manualset3
97904	8	400941	13	NULL	NULL	0	NULL	cardiogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the functional contributions of Ca ( 2 + ) transporters to ( Ca ( 2 + ) ) ( i ) decline in mouse embryonic stem cell-derived cardiomyocytes ( mESCMs ) , a suitable model for investigation of early cardiogenesis , at various differentiation stages were investigated .
	manualset3
97905	9	400941	13	NULL	NULL	0	NULL	differentiation stages 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the functional contributions of Ca ( 2 + ) transporters to ( Ca ( 2 + ) ) ( i ) decline in mouse embryonic stem cell-derived cardiomyocytes ( mESCMs ) , a suitable model for investigation of early cardiogenesis , at various differentiation stages were investigated .
	manualset3
97906	1	400942	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the mature form of glycoprotein G ( mgG-2 ) of HSV-2 was used for immunization of mice , either alone or in combination with adjuvant CpG , followed by an intravaginal challenge with a lethal dose of a fully virulent HSV-2 strain .
	manualset3
97907	2	400942	13	NULL	NULL	NULL	NULL	mature form of glycoprotein G ( mgG-2 )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , the mature form of glycoprotein G ( mgG-2 ) of HSV-2 was used for immunization of mice , either alone or in combination with adjuvant CpG , followed by an intravaginal challenge with a lethal dose of a fully virulent HSV-2 strain .
	manualset3
97908	3	400942	13	NULL	NULL	0	NULL	 HSV-2	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the mature form of glycoprotein G ( mgG-2 ) of HSV-2 was used for immunization of mice , either alone or in combination with adjuvant CpG , followed by an intravaginal challenge with a lethal dose of a fully virulent HSV-2 strain .
	manualset3
97909	4	400942	13	NULL	NULL	0	NULL	 immunization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the mature form of glycoprotein G ( mgG-2 ) of HSV-2 was used for immunization of mice , either alone or in combination with adjuvant CpG , followed by an intravaginal challenge with a lethal dose of a fully virulent HSV-2 strain .
	manualset3
97910	5	400942	13	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the mature form of glycoprotein G ( mgG-2 ) of HSV-2 was used for immunization of mice , either alone or in combination with adjuvant CpG , followed by an intravaginal challenge with a lethal dose of a fully virulent HSV-2 strain .
	manualset3
97911	6	400942	13	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the mature form of glycoprotein G ( mgG-2 ) of HSV-2 was used for immunization of mice , either alone or in combination with adjuvant CpG , followed by an intravaginal challenge with a lethal dose of a fully virulent HSV-2 strain .
	manualset3
97912	7	400942	13	NULL	NULL	0	NULL	adjuvant CpG 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the mature form of glycoprotein G ( mgG-2 ) of HSV-2 was used for immunization of mice , either alone or in combination with adjuvant CpG , followed by an intravaginal challenge with a lethal dose of a fully virulent HSV-2 strain .
	manualset3
97913	8	400942	13	NULL	NULL	0	NULL	intravaginal challenge	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the mature form of glycoprotein G ( mgG-2 ) of HSV-2 was used for immunization of mice , either alone or in combination with adjuvant CpG , followed by an intravaginal challenge with a lethal dose of a fully virulent HSV-2 strain .
	manualset3
97914	9	400942	13	NULL	NULL	0	NULL	lethal dose	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the mature form of glycoprotein G ( mgG-2 ) of HSV-2 was used for immunization of mice , either alone or in combination with adjuvant CpG , followed by an intravaginal challenge with a lethal dose of a fully virulent HSV-2 strain .
	manualset3
97915	10	400942	13	NULL	NULL	0	NULL	virulent HSV-2 strain 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the mature form of glycoprotein G ( mgG-2 ) of HSV-2 was used for immunization of mice , either alone or in combination with adjuvant CpG , followed by an intravaginal challenge with a lethal dose of a fully virulent HSV-2 strain .
	manualset3
97916	1	400943	13	NULL	NULL	0	NULL	19F NMR spectra	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	19F NMR spectra of sodium fluoride in suspensions of human erythrocytes were seen to yield separate resonances for the F - populations inside and outside the cells .
	manualset3
97917	2	400943	13	NULL	NULL	0	NULL	sodium fluoride 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	19F NMR spectra of sodium fluoride in suspensions of human erythrocytes were seen to yield separate resonances for the F - populations inside and outside the cells .
	manualset3
97918	3	400943	13	NULL	NULL	0	NULL	suspensions of human erythrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	19F NMR spectra of sodium fluoride in suspensions of human erythrocytes were seen to yield separate resonances for the F - populations inside and outside the cells .
	manualset3
97919	4	400943	13	NULL	NULL	0	NULL	 resonances	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	19F NMR spectra of sodium fluoride in suspensions of human erythrocytes were seen to yield separate resonances for the F - populations inside and outside the cells .
	manualset3
97920	5	400943	13	NULL	NULL	0	NULL	F - populations 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	19F NMR spectra of sodium fluoride in suspensions of human erythrocytes were seen to yield separate resonances for the F - populations inside and outside the cells .
	manualset3
97921	6	400943	13	NULL	NULL	0	NULL	 cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	19F NMR spectra of sodium fluoride in suspensions of human erythrocytes were seen to yield separate resonances for the F - populations inside and outside the cells .
	manualset3
97922	1	400944	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the mechanism of C. jejuni colonization in chickens was studied using four human and four poultry isolates of C. jejuni .
	manualset3
97923	2	400944	13	NULL	NULL	0	NULL	mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the mechanism of C. jejuni colonization in chickens was studied using four human and four poultry isolates of C. jejuni .
	manualset3
97924	3	400944	13	NULL	NULL	0	NULL	C. jejuni	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the mechanism of C. jejuni colonization in chickens was studied using four human and four poultry isolates of C. jejuni .
	manualset3
97925	4	400944	13	NULL	NULL	0	NULL	colonization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the mechanism of C. jejuni colonization in chickens was studied using four human and four poultry isolates of C. jejuni .
	manualset3
97926	5	400944	13	NULL	NULL	0	NULL	chickens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the mechanism of C. jejuni colonization in chickens was studied using four human and four poultry isolates of C. jejuni .
	manualset3
97927	6	400944	13	NULL	NULL	NULL	NULL	four human isolates of C. jejuni	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , the mechanism of C. jejuni colonization in chickens was studied using four human and four poultry isolates of C. jejuni .
	manualset3
97928	7	400944	13	NULL	NULL	0	NULL	four poultry isolates of C. jejuni	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the mechanism of C. jejuni colonization in chickens was studied using four human and four poultry isolates of C. jejuni .
	manualset3
97929	1	400945	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the prevalence of HGV-RNA and antibodies to E2 envelope antigen ( anti-E2 ) which is a marker of past infection , have been investigated in the samples of patients with HCV and HBV infections , and the prevalence rates were compared with the control group .
	manualset3
97930	2	400945	13	NULL	NULL	0	NULL	prevalence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the prevalence of HGV-RNA and antibodies to E2 envelope antigen ( anti-E2 ) which is a marker of past infection , have been investigated in the samples of patients with HCV and HBV infections , and the prevalence rates were compared with the control group .
	manualset3
97931	3	400945	13	NULL	NULL	0	NULL	HGV-RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the prevalence of HGV-RNA and antibodies to E2 envelope antigen ( anti-E2 ) which is a marker of past infection , have been investigated in the samples of patients with HCV and HBV infections , and the prevalence rates were compared with the control group .
	manualset3
97932	4	400945	13	NULL	NULL	0	NULL	antibodies 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the prevalence of HGV-RNA and antibodies to E2 envelope antigen ( anti-E2 ) which is a marker of past infection , have been investigated in the samples of patients with HCV and HBV infections , and the prevalence rates were compared with the control group .
	manualset3
97933	5	400945	13	NULL	NULL	0	NULL	E2 envelope antigen ( anti-E2 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the prevalence of HGV-RNA and antibodies to E2 envelope antigen ( anti-E2 ) which is a marker of past infection , have been investigated in the samples of patients with HCV and HBV infections , and the prevalence rates were compared with the control group .
	manualset3
97934	6	400945	13	NULL	NULL	0	NULL	marker of past infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the prevalence of HGV-RNA and antibodies to E2 envelope antigen ( anti-E2 ) which is a marker of past infection , have been investigated in the samples of patients with HCV and HBV infections , and the prevalence rates were compared with the control group .
	manualset3
97935	7	400945	13	NULL	NULL	0	NULL	samples	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the prevalence of HGV-RNA and antibodies to E2 envelope antigen ( anti-E2 ) which is a marker of past infection , have been investigated in the samples of patients with HCV and HBV infections , and the prevalence rates were compared with the control group .
	manualset3
97936	8	400945	13	NULL	NULL	0	NULL	 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the prevalence of HGV-RNA and antibodies to E2 envelope antigen ( anti-E2 ) which is a marker of past infection , have been investigated in the samples of patients with HCV and HBV infections , and the prevalence rates were compared with the control group .
	manualset3
97937	9	400945	13	NULL	NULL	0	NULL	HCV infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the prevalence of HGV-RNA and antibodies to E2 envelope antigen ( anti-E2 ) which is a marker of past infection , have been investigated in the samples of patients with HCV and HBV infections , and the prevalence rates were compared with the control group .
	manualset3
97938	10	400945	13	NULL	NULL	0	NULL	HBV infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the prevalence of HGV-RNA and antibodies to E2 envelope antigen ( anti-E2 ) which is a marker of past infection , have been investigated in the samples of patients with HCV and HBV infections , and the prevalence rates were compared with the control group .
	manualset3
97939	11	400945	13	NULL	NULL	0	NULL	 prevalence rates	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the prevalence of HGV-RNA and antibodies to E2 envelope antigen ( anti-E2 ) which is a marker of past infection , have been investigated in the samples of patients with HCV and HBV infections , and the prevalence rates were compared with the control group .
	manualset3
97940	12	400945	13	NULL	NULL	0	NULL	control group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the prevalence of HGV-RNA and antibodies to E2 envelope antigen ( anti-E2 ) which is a marker of past infection , have been investigated in the samples of patients with HCV and HBV infections , and the prevalence rates were compared with the control group .
	manualset3
97941	1	400946	13	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the resistance of liquefied-petroleum gas ( LPG ) tanks produced from carbon steel sheet metal of different thicknesses has been investigated by bursting pressure experiments and non-linear Finite Element Method ( FEM ) method by increasing internal pressure values .
	manualset3
97942	2	400946	13	NULL	NULL	0	NULL	resistance	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the resistance of liquefied-petroleum gas ( LPG ) tanks produced from carbon steel sheet metal of different thicknesses has been investigated by bursting pressure experiments and non-linear Finite Element Method ( FEM ) method by increasing internal pressure values .
	manualset3
97943	3	400946	13	NULL	NULL	0	NULL	liquefied-petroleum gas ( LPG ) tanks	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the resistance of liquefied-petroleum gas ( LPG ) tanks produced from carbon steel sheet metal of different thicknesses has been investigated by bursting pressure experiments and non-linear Finite Element Method ( FEM ) method by increasing internal pressure values .
	manualset3
97944	4	400946	13	NULL	NULL	0	NULL	carbon steel sheet metal	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the resistance of liquefied-petroleum gas ( LPG ) tanks produced from carbon steel sheet metal of different thicknesses has been investigated by bursting pressure experiments and non-linear Finite Element Method ( FEM ) method by increasing internal pressure values .
	manualset3
97945	5	400946	13	NULL	NULL	0	NULL	different thicknesses	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the resistance of liquefied-petroleum gas ( LPG ) tanks produced from carbon steel sheet metal of different thicknesses has been investigated by bursting pressure experiments and non-linear Finite Element Method ( FEM ) method by increasing internal pressure values .
	manualset3
97946	6	400946	13	NULL	NULL	0	NULL	bursting pressure experiments 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the resistance of liquefied-petroleum gas ( LPG ) tanks produced from carbon steel sheet metal of different thicknesses has been investigated by bursting pressure experiments and non-linear Finite Element Method ( FEM ) method by increasing internal pressure values .
	manualset3
97947	7	400946	13	NULL	NULL	0	NULL	non-linear Finite Element Method ( FEM ) method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the resistance of liquefied-petroleum gas ( LPG ) tanks produced from carbon steel sheet metal of different thicknesses has been investigated by bursting pressure experiments and non-linear Finite Element Method ( FEM ) method by increasing internal pressure values .
	manualset3
97948	8	400946	13	NULL	NULL	0	NULL	 internal pressure values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the resistance of liquefied-petroleum gas ( LPG ) tanks produced from carbon steel sheet metal of different thicknesses has been investigated by bursting pressure experiments and non-linear Finite Element Method ( FEM ) method by increasing internal pressure values .
	manualset3
97949	1	400947	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the same conditions were used to depict the changes in exogenous DNA delivery in these regions .
	manualset3
97950	2	400947	13	NULL	NULL	0	NULL	conditions 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the same conditions were used to depict the changes in exogenous DNA delivery in these regions .
	manualset3
97951	3	400947	13	NULL	NULL	0	NULL	changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the same conditions were used to depict the changes in exogenous DNA delivery in these regions .
	manualset3
97952	4	400947	13	NULL	NULL	0	NULL	exogenous DNA delivery	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the same conditions were used to depict the changes in exogenous DNA delivery in these regions .
	manualset3
97953	5	400947	13	NULL	NULL	0	NULL	regions	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the same conditions were used to depict the changes in exogenous DNA delivery in these regions .
	manualset3
97954	1	400948	13	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the technique of voxel-based morphometry ( VBM ) was applied to 3-D MRI data in ALS patients to localize regional gray and white matter changes .
	manualset3
97955	2	400948	13	NULL	NULL	0	NULL	technique of voxel-based morphometry ( VBM )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the technique of voxel-based morphometry ( VBM ) was applied to 3-D MRI data in ALS patients to localize regional gray and white matter changes .
	manualset3
97956	3	400948	13	NULL	NULL	0	NULL	3-D MRI data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the technique of voxel-based morphometry ( VBM ) was applied to 3-D MRI data in ALS patients to localize regional gray and white matter changes .
	manualset3
97957	4	400948	13	NULL	NULL	0	NULL	ALS patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the technique of voxel-based morphometry ( VBM ) was applied to 3-D MRI data in ALS patients to localize regional gray and white matter changes .
	manualset3
97958	5	400948	13	NULL	NULL	0	NULL	gray matter changes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the technique of voxel-based morphometry ( VBM ) was applied to 3-D MRI data in ALS patients to localize regional gray and white matter changes .
	manualset3
97959	6	400948	13	NULL	NULL	0	NULL	white matter changes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the technique of voxel-based morphometry ( VBM ) was applied to 3-D MRI data in ALS patients to localize regional gray and white matter changes .
	manualset3
97960	1	400949	13	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , two samples found to contain malignant cells were cloudy or turbid .
	manualset3
97961	2	400949	13	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , two samples found to contain malignant cells were cloudy or turbid .
	manualset3
97962	3	400949	13	NULL	NULL	0	NULL	samples	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , two samples found to contain malignant cells were cloudy or turbid .
	manualset3
97963	4	400949	13	NULL	NULL	0	NULL	malignant cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , two samples found to contain malignant cells were cloudy or turbid .
	manualset3
97964	1	400950	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we added Mg2 + ( 0.44-1 .1 mM ) or putrescine ( approximately 0.4 mM ) to the intracellular milieu where endogenous polyamines remained , and then examined outward IRK1 currents using the whole-cell patch-clamp method at 5.4 mM external K + .
	manualset3
97965	2	400950	13	NULL	NULL	0	NULL	Mg2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we added Mg2 + ( 0.44-1 .1 mM ) or putrescine ( approximately 0.4 mM ) to the intracellular milieu where endogenous polyamines remained , and then examined outward IRK1 currents using the whole-cell patch-clamp method at 5.4 mM external K + .
	manualset3
97966	3	400950	13	NULL	NULL	0	NULL	0.44-1 .1 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we added Mg2 + ( 0.44-1 .1 mM ) or putrescine ( approximately 0.4 mM ) to the intracellular milieu where endogenous polyamines remained , and then examined outward IRK1 currents using the whole-cell patch-clamp method at 5.4 mM external K + .
	manualset3
97967	4	400950	13	NULL	NULL	0	NULL	putrescine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we added Mg2 + ( 0.44-1 .1 mM ) or putrescine ( approximately 0.4 mM ) to the intracellular milieu where endogenous polyamines remained , and then examined outward IRK1 currents using the whole-cell patch-clamp method at 5.4 mM external K + .
	manualset3
97968	5	400950	13	NULL	NULL	0	NULL	approximately 0.4 mM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we added Mg2 + ( 0.44-1 .1 mM ) or putrescine ( approximately 0.4 mM ) to the intracellular milieu where endogenous polyamines remained , and then examined outward IRK1 currents using the whole-cell patch-clamp method at 5.4 mM external K + .
	manualset3
97969	6	400950	13	NULL	NULL	0	NULL	 intracellular milieu	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we added Mg2 + ( 0.44-1 .1 mM ) or putrescine ( approximately 0.4 mM ) to the intracellular milieu where endogenous polyamines remained , and then examined outward IRK1 currents using the whole-cell patch-clamp method at 5.4 mM external K + .
	manualset3
97970	7	400950	13	NULL	NULL	0	NULL	polyamines	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we added Mg2 + ( 0.44-1 .1 mM ) or putrescine ( approximately 0.4 mM ) to the intracellular milieu where endogenous polyamines remained , and then examined outward IRK1 currents using the whole-cell patch-clamp method at 5.4 mM external K + .
	manualset3
97971	8	400950	13	NULL	NULL	0	NULL	IRK1 currents	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we added Mg2 + ( 0.44-1 .1 mM ) or putrescine ( approximately 0.4 mM ) to the intracellular milieu where endogenous polyamines remained , and then examined outward IRK1 currents using the whole-cell patch-clamp method at 5.4 mM external K + .
	manualset3
97972	9	400950	13	NULL	NULL	0	NULL	whole-cell patch-clamp method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we added Mg2 + ( 0.44-1 .1 mM ) or putrescine ( approximately 0.4 mM ) to the intracellular milieu where endogenous polyamines remained , and then examined outward IRK1 currents using the whole-cell patch-clamp method at 5.4 mM external K + .
	manualset3
97973	10	400950	13	NULL	NULL	0	NULL	5.4 mM external K +	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we added Mg2 + ( 0.44-1 .1 mM ) or putrescine ( approximately 0.4 mM ) to the intracellular milieu where endogenous polyamines remained , and then examined outward IRK1 currents using the whole-cell patch-clamp method at 5.4 mM external K + .
	manualset3
97974	1	400951	13	NULL	NULL	0	NULL	1H-NMR studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	1H-NMR studies on a potent and selective antagonist at human melanocortin receptor 4 ( hMC-4R ) .
	manualset3
97975	2	400951	13	NULL	NULL	NULL	NULL	potent and selective antagonist	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	1H-NMR studies on a potent and selective antagonist at human melanocortin receptor 4 ( hMC-4R ) .
	manualset3
97977	4	400951	13	NULL	NULL	0	NULL	human melanocortin receptor 4 ( hMC-4R )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	1H-NMR studies on a potent and selective antagonist at human melanocortin receptor 4 ( hMC-4R ) .
	manualset3
97978	1	400952	13	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we aimed to identify CYPs that are up-regulated during keratinocyte differentiation and potentially responsible for epoxyeicosatrienoic acid formation in human skin .
	manualset3
97979	2	400952	13	NULL	NULL	0	NULL	 CYPs 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we aimed to identify CYPs that are up-regulated during keratinocyte differentiation and potentially responsible for epoxyeicosatrienoic acid formation in human skin .
	manualset3
97980	3	400952	13	NULL	NULL	0	NULL	keratinocyte differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we aimed to identify CYPs that are up-regulated during keratinocyte differentiation and potentially responsible for epoxyeicosatrienoic acid formation in human skin .
	manualset3
97981	4	400952	13	NULL	NULL	0	NULL	epoxyeicosatrienoic acid formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we aimed to identify CYPs that are up-regulated during keratinocyte differentiation and potentially responsible for epoxyeicosatrienoic acid formation in human skin .
	manualset3
97982	5	400952	13	NULL	NULL	0	NULL	human skin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we aimed to identify CYPs that are up-regulated during keratinocyte differentiation and potentially responsible for epoxyeicosatrienoic acid formation in human skin .
	manualset3
97983	1	400953	13	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we assessed the clinical characteristics and IVUS findings of patients whose CFR remained below 2.0 after stent implantation , specifically 16 patients with CFR below 2.0 ( 22 lesions , 64 + / - 9 years , 4 female ) , and 102 patients with CFR above 2.0 ( 112 lesions , mean age 66 + / - 11 years , 22 female ) .
	manualset3
97984	2	400953	13	NULL	NULL	0	NULL	clinical characteristics 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we assessed the clinical characteristics and IVUS findings of patients whose CFR remained below 2.0 after stent implantation , specifically 16 patients with CFR below 2.0 ( 22 lesions , 64 + / - 9 years , 4 female ) , and 102 patients with CFR above 2.0 ( 112 lesions , mean age 66 + / - 11 years , 22 female ) .
	manualset3
97985	3	400953	13	NULL	NULL	0	NULL	 IVUS findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we assessed the clinical characteristics and IVUS findings of patients whose CFR remained below 2.0 after stent implantation , specifically 16 patients with CFR below 2.0 ( 22 lesions , 64 + / - 9 years , 4 female ) , and 102 patients with CFR above 2.0 ( 112 lesions , mean age 66 + / - 11 years , 22 female ) .
	manualset3
97986	4	400953	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we assessed the clinical characteristics and IVUS findings of patients whose CFR remained below 2.0 after stent implantation , specifically 16 patients with CFR below 2.0 ( 22 lesions , 64 + / - 9 years , 4 female ) , and 102 patients with CFR above 2.0 ( 112 lesions , mean age 66 + / - 11 years , 22 female ) .
	manualset3
97987	5	400953	13	NULL	NULL	0	NULL	CFR 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we assessed the clinical characteristics and IVUS findings of patients whose CFR remained below 2.0 after stent implantation , specifically 16 patients with CFR below 2.0 ( 22 lesions , 64 + / - 9 years , 4 female ) , and 102 patients with CFR above 2.0 ( 112 lesions , mean age 66 + / - 11 years , 22 female ) .
	manualset3
97988	6	400953	13	NULL	NULL	0	NULL	below 2.0	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we assessed the clinical characteristics and IVUS findings of patients whose CFR remained below 2.0 after stent implantation , specifically 16 patients with CFR below 2.0 ( 22 lesions , 64 + / - 9 years , 4 female ) , and 102 patients with CFR above 2.0 ( 112 lesions , mean age 66 + / - 11 years , 22 female ) .
	manualset3
97989	7	400953	13	NULL	NULL	0	NULL	stent implantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we assessed the clinical characteristics and IVUS findings of patients whose CFR remained below 2.0 after stent implantation , specifically 16 patients with CFR below 2.0 ( 22 lesions , 64 + / - 9 years , 4 female ) , and 102 patients with CFR above 2.0 ( 112 lesions , mean age 66 + / - 11 years , 22 female ) .
	manualset3
97990	8	400953	13	NULL	NULL	0	NULL	16 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we assessed the clinical characteristics and IVUS findings of patients whose CFR remained below 2.0 after stent implantation , specifically 16 patients with CFR below 2.0 ( 22 lesions , 64 + / - 9 years , 4 female ) , and 102 patients with CFR above 2.0 ( 112 lesions , mean age 66 + / - 11 years , 22 female ) .
	manualset3
97991	9	400953	13	NULL	NULL	0	NULL	CFR	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we assessed the clinical characteristics and IVUS findings of patients whose CFR remained below 2.0 after stent implantation , specifically 16 patients with CFR below 2.0 ( 22 lesions , 64 + / - 9 years , 4 female ) , and 102 patients with CFR above 2.0 ( 112 lesions , mean age 66 + / - 11 years , 22 female ) .
	manualset3
97992	10	400953	13	NULL	NULL	0	NULL	below 2.0 ( 22 lesions , 64 + / - 9 years , 4 female )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we assessed the clinical characteristics and IVUS findings of patients whose CFR remained below 2.0 after stent implantation , specifically 16 patients with CFR below 2.0 ( 22 lesions , 64 + / - 9 years , 4 female ) , and 102 patients with CFR above 2.0 ( 112 lesions , mean age 66 + / - 11 years , 22 female ) .
	manualset3
97993	11	400953	13	NULL	NULL	0	NULL	102 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we assessed the clinical characteristics and IVUS findings of patients whose CFR remained below 2.0 after stent implantation , specifically 16 patients with CFR below 2.0 ( 22 lesions , 64 + / - 9 years , 4 female ) , and 102 patients with CFR above 2.0 ( 112 lesions , mean age 66 + / - 11 years , 22 female ) .
	manualset3
97994	12	400953	13	NULL	NULL	0	NULL	CFR	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we assessed the clinical characteristics and IVUS findings of patients whose CFR remained below 2.0 after stent implantation , specifically 16 patients with CFR below 2.0 ( 22 lesions , 64 + / - 9 years , 4 female ) , and 102 patients with CFR above 2.0 ( 112 lesions , mean age 66 + / - 11 years , 22 female ) .
	manualset3
97995	13	400953	13	NULL	NULL	0	NULL	above 2.0 ( 112 lesions , mean age 66 + / - 11 years , 22 female ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we assessed the clinical characteristics and IVUS findings of patients whose CFR remained below 2.0 after stent implantation , specifically 16 patients with CFR below 2.0 ( 22 lesions , 64 + / - 9 years , 4 female ) , and 102 patients with CFR above 2.0 ( 112 lesions , mean age 66 + / - 11 years , 22 female ) .
	manualset3
97996	1	400954	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we built a cattle phylogeny with a pool of 856 individual D-loop sequences , of which 264 Chinese cattle D-loop sequences were obtained in this study ( 141 ones were first analyzed , and 123 were first submitted ) and the rest sequences of cattle from six Asian countries ( Japan , Korea , Mongolia , Nepal , India and China ) were retrieved from GenBank .
	manualset3
97997	2	400954	13	NULL	NULL	NULL	NULL	cattle phylogeny	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , we built a cattle phylogeny with a pool of 856 individual D-loop sequences , of which 264 Chinese cattle D-loop sequences were obtained in this study ( 141 ones were first analyzed , and 123 were first submitted ) and the rest sequences of cattle from six Asian countries ( Japan , Korea , Mongolia , Nepal , India and China ) were retrieved from GenBank .
	manualset3
97998	3	400954	13	NULL	NULL	0	NULL	 pool of 856 individual D-loop sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we built a cattle phylogeny with a pool of 856 individual D-loop sequences , of which 264 Chinese cattle D-loop sequences were obtained in this study ( 141 ones were first analyzed , and 123 were first submitted ) and the rest sequences of cattle from six Asian countries ( Japan , Korea , Mongolia , Nepal , India and China ) were retrieved from GenBank .
	manualset3
97999	4	400954	13	NULL	NULL	0	NULL	264 Chinese cattle D-loop sequences 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we built a cattle phylogeny with a pool of 856 individual D-loop sequences , of which 264 Chinese cattle D-loop sequences were obtained in this study ( 141 ones were first analyzed , and 123 were first submitted ) and the rest sequences of cattle from six Asian countries ( Japan , Korea , Mongolia , Nepal , India and China ) were retrieved from GenBank .
	manualset3
98000	5	400954	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we built a cattle phylogeny with a pool of 856 individual D-loop sequences , of which 264 Chinese cattle D-loop sequences were obtained in this study ( 141 ones were first analyzed , and 123 were first submitted ) and the rest sequences of cattle from six Asian countries ( Japan , Korea , Mongolia , Nepal , India and China ) were retrieved from GenBank .
	manualset3
98001	6	400954	13	NULL	NULL	NULL	NULL	141 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , we built a cattle phylogeny with a pool of 856 individual D-loop sequences , of which 264 Chinese cattle D-loop sequences were obtained in this study ( 141 ones were first analyzed , and 123 were first submitted ) and the rest sequences of cattle from six Asian countries ( Japan , Korea , Mongolia , Nepal , India and China ) were retrieved from GenBank .
	manualset3
98002	7	400954	13	NULL	NULL	0	NULL	123 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we built a cattle phylogeny with a pool of 856 individual D-loop sequences , of which 264 Chinese cattle D-loop sequences were obtained in this study ( 141 ones were first analyzed , and 123 were first submitted ) and the rest sequences of cattle from six Asian countries ( Japan , Korea , Mongolia , Nepal , India and China ) were retrieved from GenBank .
	manualset3
98003	8	400954	13	NULL	NULL	0	NULL	sequences of cattle	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we built a cattle phylogeny with a pool of 856 individual D-loop sequences , of which 264 Chinese cattle D-loop sequences were obtained in this study ( 141 ones were first analyzed , and 123 were first submitted ) and the rest sequences of cattle from six Asian countries ( Japan , Korea , Mongolia , Nepal , India and China ) were retrieved from GenBank .
	manualset3
98004	9	400954	13	NULL	NULL	NULL	NULL	six Asian countries	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , we built a cattle phylogeny with a pool of 856 individual D-loop sequences , of which 264 Chinese cattle D-loop sequences were obtained in this study ( 141 ones were first analyzed , and 123 were first submitted ) and the rest sequences of cattle from six Asian countries ( Japan , Korea , Mongolia , Nepal , India and China ) were retrieved from GenBank .
	manualset3
98005	10	400954	13	NULL	NULL	0	NULL	Japan	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we built a cattle phylogeny with a pool of 856 individual D-loop sequences , of which 264 Chinese cattle D-loop sequences were obtained in this study ( 141 ones were first analyzed , and 123 were first submitted ) and the rest sequences of cattle from six Asian countries ( Japan , Korea , Mongolia , Nepal , India and China ) were retrieved from GenBank .
	manualset3
98006	11	400954	13	NULL	NULL	0	NULL	Korea	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we built a cattle phylogeny with a pool of 856 individual D-loop sequences , of which 264 Chinese cattle D-loop sequences were obtained in this study ( 141 ones were first analyzed , and 123 were first submitted ) and the rest sequences of cattle from six Asian countries ( Japan , Korea , Mongolia , Nepal , India and China ) were retrieved from GenBank .
	manualset3
98007	12	400954	13	NULL	NULL	0	NULL	Mongolia	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we built a cattle phylogeny with a pool of 856 individual D-loop sequences , of which 264 Chinese cattle D-loop sequences were obtained in this study ( 141 ones were first analyzed , and 123 were first submitted ) and the rest sequences of cattle from six Asian countries ( Japan , Korea , Mongolia , Nepal , India and China ) were retrieved from GenBank .
	manualset3
98008	13	400954	13	NULL	NULL	0	NULL	Nepal 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we built a cattle phylogeny with a pool of 856 individual D-loop sequences , of which 264 Chinese cattle D-loop sequences were obtained in this study ( 141 ones were first analyzed , and 123 were first submitted ) and the rest sequences of cattle from six Asian countries ( Japan , Korea , Mongolia , Nepal , India and China ) were retrieved from GenBank .
	manualset3
98009	14	400954	13	NULL	NULL	0	NULL	India	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we built a cattle phylogeny with a pool of 856 individual D-loop sequences , of which 264 Chinese cattle D-loop sequences were obtained in this study ( 141 ones were first analyzed , and 123 were first submitted ) and the rest sequences of cattle from six Asian countries ( Japan , Korea , Mongolia , Nepal , India and China ) were retrieved from GenBank .
	manualset3
98010	15	400954	13	NULL	NULL	0	NULL	China	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we built a cattle phylogeny with a pool of 856 individual D-loop sequences , of which 264 Chinese cattle D-loop sequences were obtained in this study ( 141 ones were first analyzed , and 123 were first submitted ) and the rest sequences of cattle from six Asian countries ( Japan , Korea , Mongolia , Nepal , India and China ) were retrieved from GenBank .
	manualset3
98011	16	400954	13	NULL	NULL	0	NULL	GenBank	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we built a cattle phylogeny with a pool of 856 individual D-loop sequences , of which 264 Chinese cattle D-loop sequences were obtained in this study ( 141 ones were first analyzed , and 123 were first submitted ) and the rest sequences of cattle from six Asian countries ( Japan , Korea , Mongolia , Nepal , India and China ) were retrieved from GenBank .
	manualset3
98012	1	400955	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we carried out derivatization for 6FP and succeeded in increasing water solubility with maintaining its physiological activities .
	manualset3
98013	2	400955	13	NULL	NULL	0	NULL	derivatization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we carried out derivatization for 6FP and succeeded in increasing water solubility with maintaining its physiological activities .
	manualset3
98014	3	400955	13	NULL	NULL	0	NULL	6FP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we carried out derivatization for 6FP and succeeded in increasing water solubility with maintaining its physiological activities .
	manualset3
98015	4	400955	13	NULL	NULL	0	NULL	water solubility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we carried out derivatization for 6FP and succeeded in increasing water solubility with maintaining its physiological activities .
	manualset3
98016	5	400955	13	NULL	NULL	0	NULL	physiological activities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we carried out derivatization for 6FP and succeeded in increasing water solubility with maintaining its physiological activities .
	manualset3
98017	1	400956	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we characterized the molecular mechanisms by which quercetin and its enteric bacterial metabolites , taxifolin , alphitonin , and 3 , 4-dihydroxy-phenylacetic acid , inhibit tumor necrosis factor alpha ( TNF ) - induced proinflammatory gene expression in the murine small intestinal epithelial cell ( IEC ) line Mode-K as well as in heterozygous TNFDeltaARE/WT mice , a murine model of experimental ileitis .
	manualset3
98018	2	400956	13	NULL	NULL	0	NULL	 molecular mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we characterized the molecular mechanisms by which quercetin and its enteric bacterial metabolites , taxifolin , alphitonin , and 3 , 4-dihydroxy-phenylacetic acid , inhibit tumor necrosis factor alpha ( TNF ) - induced proinflammatory gene expression in the murine small intestinal epithelial cell ( IEC ) line Mode-K as well as in heterozygous TNFDeltaARE/WT mice , a murine model of experimental ileitis .
	manualset3
98019	3	400956	13	NULL	NULL	0	NULL	quercetin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we characterized the molecular mechanisms by which quercetin and its enteric bacterial metabolites , taxifolin , alphitonin , and 3 , 4-dihydroxy-phenylacetic acid , inhibit tumor necrosis factor alpha ( TNF ) - induced proinflammatory gene expression in the murine small intestinal epithelial cell ( IEC ) line Mode-K as well as in heterozygous TNFDeltaARE/WT mice , a murine model of experimental ileitis .
	manualset3
98020	4	400956	13	NULL	NULL	0	NULL	enteric bacterial metabolites 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we characterized the molecular mechanisms by which quercetin and its enteric bacterial metabolites , taxifolin , alphitonin , and 3 , 4-dihydroxy-phenylacetic acid , inhibit tumor necrosis factor alpha ( TNF ) - induced proinflammatory gene expression in the murine small intestinal epithelial cell ( IEC ) line Mode-K as well as in heterozygous TNFDeltaARE/WT mice , a murine model of experimental ileitis .
	manualset3
98021	5	400956	13	NULL	NULL	0	NULL	taxifolin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we characterized the molecular mechanisms by which quercetin and its enteric bacterial metabolites , taxifolin , alphitonin , and 3 , 4-dihydroxy-phenylacetic acid , inhibit tumor necrosis factor alpha ( TNF ) - induced proinflammatory gene expression in the murine small intestinal epithelial cell ( IEC ) line Mode-K as well as in heterozygous TNFDeltaARE/WT mice , a murine model of experimental ileitis .
	manualset3
98022	6	400956	13	NULL	NULL	0	NULL	alphitonin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we characterized the molecular mechanisms by which quercetin and its enteric bacterial metabolites , taxifolin , alphitonin , and 3 , 4-dihydroxy-phenylacetic acid , inhibit tumor necrosis factor alpha ( TNF ) - induced proinflammatory gene expression in the murine small intestinal epithelial cell ( IEC ) line Mode-K as well as in heterozygous TNFDeltaARE/WT mice , a murine model of experimental ileitis .
	manualset3
98023	7	400956	13	NULL	NULL	0	NULL	3 , 4-dihydroxy-phenylacetic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we characterized the molecular mechanisms by which quercetin and its enteric bacterial metabolites , taxifolin , alphitonin , and 3 , 4-dihydroxy-phenylacetic acid , inhibit tumor necrosis factor alpha ( TNF ) - induced proinflammatory gene expression in the murine small intestinal epithelial cell ( IEC ) line Mode-K as well as in heterozygous TNFDeltaARE/WT mice , a murine model of experimental ileitis .
	manualset3
98024	8	400956	13	NULL	NULL	0	NULL	tumor necrosis factor alpha ( TNF ) - induced proinflammatory gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we characterized the molecular mechanisms by which quercetin and its enteric bacterial metabolites , taxifolin , alphitonin , and 3 , 4-dihydroxy-phenylacetic acid , inhibit tumor necrosis factor alpha ( TNF ) - induced proinflammatory gene expression in the murine small intestinal epithelial cell ( IEC ) line Mode-K as well as in heterozygous TNFDeltaARE/WT mice , a murine model of experimental ileitis .
	manualset3
98025	9	400956	13	NULL	NULL	0	NULL	 murine small intestinal epithelial cell ( IEC ) line Mode-K	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we characterized the molecular mechanisms by which quercetin and its enteric bacterial metabolites , taxifolin , alphitonin , and 3 , 4-dihydroxy-phenylacetic acid , inhibit tumor necrosis factor alpha ( TNF ) - induced proinflammatory gene expression in the murine small intestinal epithelial cell ( IEC ) line Mode-K as well as in heterozygous TNFDeltaARE/WT mice , a murine model of experimental ileitis .
	manualset3
98026	10	400956	13	NULL	NULL	0	NULL	heterozygous TNFDeltaARE/WT mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we characterized the molecular mechanisms by which quercetin and its enteric bacterial metabolites , taxifolin , alphitonin , and 3 , 4-dihydroxy-phenylacetic acid , inhibit tumor necrosis factor alpha ( TNF ) - induced proinflammatory gene expression in the murine small intestinal epithelial cell ( IEC ) line Mode-K as well as in heterozygous TNFDeltaARE/WT mice , a murine model of experimental ileitis .
	manualset3
98027	11	400956	13	NULL	NULL	0	NULL	murine model of experimental ileitis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we characterized the molecular mechanisms by which quercetin and its enteric bacterial metabolites , taxifolin , alphitonin , and 3 , 4-dihydroxy-phenylacetic acid , inhibit tumor necrosis factor alpha ( TNF ) - induced proinflammatory gene expression in the murine small intestinal epithelial cell ( IEC ) line Mode-K as well as in heterozygous TNFDeltaARE/WT mice , a murine model of experimental ileitis .
	manualset3
98028	1	400957	13	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we collected DNA samples from 480 Taiwanese subjects ( 189 calcium nephrolithiasis patients and 291 controls ) for genotyping the CASR gene .
	manualset3
98029	2	400957	13	NULL	NULL	0	NULL	 DNA samples	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we collected DNA samples from 480 Taiwanese subjects ( 189 calcium nephrolithiasis patients and 291 controls ) for genotyping the CASR gene .
	manualset3
98030	3	400957	13	NULL	NULL	0	NULL	480 Taiwanese subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we collected DNA samples from 480 Taiwanese subjects ( 189 calcium nephrolithiasis patients and 291 controls ) for genotyping the CASR gene .
	manualset3
98031	4	400957	13	NULL	NULL	0	NULL	189 calcium nephrolithiasis patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we collected DNA samples from 480 Taiwanese subjects ( 189 calcium nephrolithiasis patients and 291 controls ) for genotyping the CASR gene .
	manualset3
98032	5	400957	13	NULL	NULL	0	NULL	291 controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we collected DNA samples from 480 Taiwanese subjects ( 189 calcium nephrolithiasis patients and 291 controls ) for genotyping the CASR gene .
	manualset3
98033	6	400957	13	NULL	NULL	0	NULL	CASR gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we collected DNA samples from 480 Taiwanese subjects ( 189 calcium nephrolithiasis patients and 291 controls ) for genotyping the CASR gene .
	manualset3
98034	1	400958	13	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we demonstrate that , like UHRF1 , UHRF2 also binds preferentially to methylated histone H3 lysine 9 ( H3K9 ) through its conserved tudor domain and hemi-methylated DNA through the SET and Ring associated domain .
	manualset3
98035	2	400958	13	NULL	NULL	0	NULL	UHRF1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we demonstrate that , like UHRF1 , UHRF2 also binds preferentially to methylated histone H3 lysine 9 ( H3K9 ) through its conserved tudor domain and hemi-methylated DNA through the SET and Ring associated domain .
	manualset3
98036	3	400958	13	NULL	NULL	0	NULL	UHRF2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we demonstrate that , like UHRF1 , UHRF2 also binds preferentially to methylated histone H3 lysine 9 ( H3K9 ) through its conserved tudor domain and hemi-methylated DNA through the SET and Ring associated domain .
	manualset3
98037	4	400958	13	NULL	NULL	0	NULL	histone H3 lysine 9 ( H3K9 )	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we demonstrate that , like UHRF1 , UHRF2 also binds preferentially to methylated histone H3 lysine 9 ( H3K9 ) through its conserved tudor domain and hemi-methylated DNA through the SET and Ring associated domain .
	manualset3
98038	5	400958	13	NULL	NULL	0	NULL	tudor domain 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we demonstrate that , like UHRF1 , UHRF2 also binds preferentially to methylated histone H3 lysine 9 ( H3K9 ) through its conserved tudor domain and hemi-methylated DNA through the SET and Ring associated domain .
	manualset3
98039	6	400958	13	NULL	NULL	0	NULL	hemi-methylated DNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we demonstrate that , like UHRF1 , UHRF2 also binds preferentially to methylated histone H3 lysine 9 ( H3K9 ) through its conserved tudor domain and hemi-methylated DNA through the SET and Ring associated domain .
	manualset3
98040	7	400958	13	NULL	NULL	0	NULL	 SET	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we demonstrate that , like UHRF1 , UHRF2 also binds preferentially to methylated histone H3 lysine 9 ( H3K9 ) through its conserved tudor domain and hemi-methylated DNA through the SET and Ring associated domain .
	manualset3
98041	8	400958	13	NULL	NULL	0	NULL	Ring associated domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we demonstrate that , like UHRF1 , UHRF2 also binds preferentially to methylated histone H3 lysine 9 ( H3K9 ) through its conserved tudor domain and hemi-methylated DNA through the SET and Ring associated domain .
	manualset3
98042	1	400959	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we demonstrate that ear mesenchymal stem cells ( EMSC ) express stromal cell-associated markers ( CD44 , CD73 ) and stem cell marker Sca-1 and can be differentiated into spontaneously contracting muscle cells .
	manualset3
98043	2	400959	13	NULL	NULL	0	NULL	ear mesenchymal stem cells ( EMSC )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we demonstrate that ear mesenchymal stem cells ( EMSC ) express stromal cell-associated markers ( CD44 , CD73 ) and stem cell marker Sca-1 and can be differentiated into spontaneously contracting muscle cells .
	manualset3
98044	3	400959	13	NULL	NULL	0	NULL	stromal cell-associated markers 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we demonstrate that ear mesenchymal stem cells ( EMSC ) express stromal cell-associated markers ( CD44 , CD73 ) and stem cell marker Sca-1 and can be differentiated into spontaneously contracting muscle cells .
	manualset3
98045	4	400959	13	NULL	NULL	0	NULL	CD44	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we demonstrate that ear mesenchymal stem cells ( EMSC ) express stromal cell-associated markers ( CD44 , CD73 ) and stem cell marker Sca-1 and can be differentiated into spontaneously contracting muscle cells .
	manualset3
98046	5	400959	13	NULL	NULL	0	NULL	CD73 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we demonstrate that ear mesenchymal stem cells ( EMSC ) express stromal cell-associated markers ( CD44 , CD73 ) and stem cell marker Sca-1 and can be differentiated into spontaneously contracting muscle cells .
	manualset3
98047	6	400959	13	NULL	NULL	0	NULL	stem cell marker Sca-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we demonstrate that ear mesenchymal stem cells ( EMSC ) express stromal cell-associated markers ( CD44 , CD73 ) and stem cell marker Sca-1 and can be differentiated into spontaneously contracting muscle cells .
	manualset3
98048	7	400959	13	NULL	NULL	0	NULL	muscle cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we demonstrate that ear mesenchymal stem cells ( EMSC ) express stromal cell-associated markers ( CD44 , CD73 ) and stem cell marker Sca-1 and can be differentiated into spontaneously contracting muscle cells .
	manualset3
98049	1	400960	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we demonstrated that the d , l-endopeptidase activity at the lateral cell wall is essential for cell proliferation .
	manualset3
98050	2	400960	13	NULL	NULL	0	NULL	d , l-endopeptidase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we demonstrated that the d , l-endopeptidase activity at the lateral cell wall is essential for cell proliferation .
	manualset3
98051	3	400960	13	NULL	NULL	0	NULL	cell wall 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we demonstrated that the d , l-endopeptidase activity at the lateral cell wall is essential for cell proliferation .
	manualset3
98052	4	400960	13	NULL	NULL	0	NULL	cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we demonstrated that the d , l-endopeptidase activity at the lateral cell wall is essential for cell proliferation .
	manualset3
98053	1	400961	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we describe the development and validation of a questionnaire to assess knowledge of information typically included in genetic counseling for breast cancer .
	manualset3
98054	2	400961	13	NULL	NULL	0	NULL	development of a questionnaire	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we describe the development and validation of a questionnaire to assess knowledge of information typically included in genetic counseling for breast cancer .
	manualset3
98055	3	400961	13	NULL	NULL	0	NULL	validation of a questionnaire	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we describe the development and validation of a questionnaire to assess knowledge of information typically included in genetic counseling for breast cancer .
	manualset3
98056	4	400961	13	NULL	NULL	0	NULL	knowledge of information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we describe the development and validation of a questionnaire to assess knowledge of information typically included in genetic counseling for breast cancer .
	manualset3
98057	5	400961	13	NULL	NULL	0	NULL	genetic counseling	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we describe the development and validation of a questionnaire to assess knowledge of information typically included in genetic counseling for breast cancer .
	manualset3
98058	6	400961	13	NULL	NULL	0	NULL	breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we describe the development and validation of a questionnaire to assess knowledge of information typically included in genetic counseling for breast cancer .
	manualset3
98059	1	400962	13	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we describe the preparation of bacteriorhodopsin ( bR ) monolayers on Br-terminated solid supports through covalent attachment .
	manualset3
98060	2	400962	13	NULL	NULL	0	NULL	preparation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we describe the preparation of bacteriorhodopsin ( bR ) monolayers on Br-terminated solid supports through covalent attachment .
	manualset3
98061	3	400962	13	NULL	NULL	0	NULL	bacteriorhodopsin ( bR ) monolayers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we describe the preparation of bacteriorhodopsin ( bR ) monolayers on Br-terminated solid supports through covalent attachment .
	manualset3
98062	4	400962	13	NULL	NULL	0	NULL	Br-terminated solid supports	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we describe the preparation of bacteriorhodopsin ( bR ) monolayers on Br-terminated solid supports through covalent attachment .
	manualset3
98063	5	400962	13	NULL	NULL	0	NULL	covalent attachment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we describe the preparation of bacteriorhodopsin ( bR ) monolayers on Br-terminated solid supports through covalent attachment .
	manualset3
98064	1	400963	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we determined whether all-trans-retinoic acid ( tRA ) and follicle-stimulating hormone ( FSH ) modulate RARalpha receptor subcellular localization , leading to changes in its transcriptional activity and protein expression in mouse Sertoli cell lines .
	manualset3
98065	2	400963	13	NULL	NULL	0	NULL	all-trans-retinoic acid ( tRA ) 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we determined whether all-trans-retinoic acid ( tRA ) and follicle-stimulating hormone ( FSH ) modulate RARalpha receptor subcellular localization , leading to changes in its transcriptional activity and protein expression in mouse Sertoli cell lines .
	manualset3
98066	3	400963	13	NULL	NULL	0	NULL	follicle-stimulating hormone ( FSH ) 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we determined whether all-trans-retinoic acid ( tRA ) and follicle-stimulating hormone ( FSH ) modulate RARalpha receptor subcellular localization , leading to changes in its transcriptional activity and protein expression in mouse Sertoli cell lines .
	manualset3
98067	4	400963	13	NULL	NULL	0	NULL	RARalpha receptor subcellular localization 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we determined whether all-trans-retinoic acid ( tRA ) and follicle-stimulating hormone ( FSH ) modulate RARalpha receptor subcellular localization , leading to changes in its transcriptional activity and protein expression in mouse Sertoli cell lines .
	manualset3
98068	5	400963	13	NULL	NULL	0	NULL	changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we determined whether all-trans-retinoic acid ( tRA ) and follicle-stimulating hormone ( FSH ) modulate RARalpha receptor subcellular localization , leading to changes in its transcriptional activity and protein expression in mouse Sertoli cell lines .
	manualset3
98069	6	400963	13	NULL	NULL	0	NULL	transcriptional activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we determined whether all-trans-retinoic acid ( tRA ) and follicle-stimulating hormone ( FSH ) modulate RARalpha receptor subcellular localization , leading to changes in its transcriptional activity and protein expression in mouse Sertoli cell lines .
	manualset3
98070	7	400963	13	NULL	NULL	0	NULL	protein expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we determined whether all-trans-retinoic acid ( tRA ) and follicle-stimulating hormone ( FSH ) modulate RARalpha receptor subcellular localization , leading to changes in its transcriptional activity and protein expression in mouse Sertoli cell lines .
	manualset3
98071	8	400963	13	NULL	NULL	0	NULL	mouse Sertoli cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we determined whether all-trans-retinoic acid ( tRA ) and follicle-stimulating hormone ( FSH ) modulate RARalpha receptor subcellular localization , leading to changes in its transcriptional activity and protein expression in mouse Sertoli cell lines .
	manualset3
98072	1	400964	13	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we developed and tested a method for human biomonitoring using Comet assays with human T - and B-lymphocytes obtained by magnetic cell sorting ( MACS ) .
	manualset3
98073	2	400964	13	NULL	NULL	0	NULL	method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we developed and tested a method for human biomonitoring using Comet assays with human T - and B-lymphocytes obtained by magnetic cell sorting ( MACS ) .
	manualset3
98074	3	400964	13	NULL	NULL	0	NULL	human biomonitoring 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we developed and tested a method for human biomonitoring using Comet assays with human T - and B-lymphocytes obtained by magnetic cell sorting ( MACS ) .
	manualset3
98075	4	400964	13	NULL	NULL	0	NULL	Comet assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we developed and tested a method for human biomonitoring using Comet assays with human T - and B-lymphocytes obtained by magnetic cell sorting ( MACS ) .
	manualset3
98076	5	400964	13	NULL	NULL	0	NULL	human T-lymphocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we developed and tested a method for human biomonitoring using Comet assays with human T - and B-lymphocytes obtained by magnetic cell sorting ( MACS ) .
	manualset3
98077	6	400964	13	NULL	NULL	0	NULL	human B-lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we developed and tested a method for human biomonitoring using Comet assays with human T - and B-lymphocytes obtained by magnetic cell sorting ( MACS ) .
	manualset3
98078	7	400964	13	NULL	NULL	0	NULL	magnetic cell sorting ( MACS ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we developed and tested a method for human biomonitoring using Comet assays with human T - and B-lymphocytes obtained by magnetic cell sorting ( MACS ) .
	manualset3
98079	1	400965	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we established a convenient and universal method for detecting MRD in DLBCL .
	manualset3
98080	2	400965	13	NULL	NULL	0	NULL	convenient method	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we established a convenient and universal method for detecting MRD in DLBCL .
	manualset3
98081	3	400965	13	NULL	NULL	0	NULL	universal method 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we established a convenient and universal method for detecting MRD in DLBCL .
	manualset3
98082	4	400965	13	NULL	NULL	0	NULL	MRD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we established a convenient and universal method for detecting MRD in DLBCL .
	manualset3
98083	5	400965	13	NULL	NULL	0	NULL	DLBCL	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we established a convenient and universal method for detecting MRD in DLBCL .
	manualset3
98084	1	400966	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we evaluated by Western blot the effects in vitro of GHRH and its antagonist JMR-132 on proliferating cell nuclear antigen , tumor suppressor protein p53 , transcription factor NF-kappaB p50 and its phosphorylated form , caspase 3 , and cleaved caspase 3 in the LNCaP human prostate cancer cell line .
	manualset3
98085	2	400966	13	NULL	NULL	0	NULL	Western blot	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we evaluated by Western blot the effects in vitro of GHRH and its antagonist JMR-132 on proliferating cell nuclear antigen , tumor suppressor protein p53 , transcription factor NF-kappaB p50 and its phosphorylated form , caspase 3 , and cleaved caspase 3 in the LNCaP human prostate cancer cell line .
	manualset3
98086	3	400966	13	NULL	NULL	NULL	NULL	effects in vitro 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , we evaluated by Western blot the effects in vitro of GHRH and its antagonist JMR-132 on proliferating cell nuclear antigen , tumor suppressor protein p53 , transcription factor NF-kappaB p50 and its phosphorylated form , caspase 3 , and cleaved caspase 3 in the LNCaP human prostate cancer cell line .
	manualset3
98087	4	400966	13	NULL	NULL	0	NULL	GHRH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we evaluated by Western blot the effects in vitro of GHRH and its antagonist JMR-132 on proliferating cell nuclear antigen , tumor suppressor protein p53 , transcription factor NF-kappaB p50 and its phosphorylated form , caspase 3 , and cleaved caspase 3 in the LNCaP human prostate cancer cell line .
	manualset3
98088	5	400966	13	NULL	NULL	0	NULL	antagonist JMR-132 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we evaluated by Western blot the effects in vitro of GHRH and its antagonist JMR-132 on proliferating cell nuclear antigen , tumor suppressor protein p53 , transcription factor NF-kappaB p50 and its phosphorylated form , caspase 3 , and cleaved caspase 3 in the LNCaP human prostate cancer cell line .
	manualset3
98089	6	400966	13	NULL	NULL	0	NULL	proliferating cell nuclear antigen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we evaluated by Western blot the effects in vitro of GHRH and its antagonist JMR-132 on proliferating cell nuclear antigen , tumor suppressor protein p53 , transcription factor NF-kappaB p50 and its phosphorylated form , caspase 3 , and cleaved caspase 3 in the LNCaP human prostate cancer cell line .
	manualset3
98090	7	400966	13	NULL	NULL	0	NULL	tumor suppressor protein p53 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we evaluated by Western blot the effects in vitro of GHRH and its antagonist JMR-132 on proliferating cell nuclear antigen , tumor suppressor protein p53 , transcription factor NF-kappaB p50 and its phosphorylated form , caspase 3 , and cleaved caspase 3 in the LNCaP human prostate cancer cell line .
	manualset3
98091	8	400966	13	NULL	NULL	0	NULL	transcription factor NF-kappaB p50 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we evaluated by Western blot the effects in vitro of GHRH and its antagonist JMR-132 on proliferating cell nuclear antigen , tumor suppressor protein p53 , transcription factor NF-kappaB p50 and its phosphorylated form , caspase 3 , and cleaved caspase 3 in the LNCaP human prostate cancer cell line .
	manualset3
98092	10	400966	13	NULL	NULL	NULL	NULL	caspase 3 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , we evaluated by Western blot the effects in vitro of GHRH and its antagonist JMR-132 on proliferating cell nuclear antigen , tumor suppressor protein p53 , transcription factor NF-kappaB p50 and its phosphorylated form , caspase 3 , and cleaved caspase 3 in the LNCaP human prostate cancer cell line .
	manualset3
98093	11	400966	13	NULL	NULL	NULL	NULL	cleaved caspase 3	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , we evaluated by Western blot the effects in vitro of GHRH and its antagonist JMR-132 on proliferating cell nuclear antigen , tumor suppressor protein p53 , transcription factor NF-kappaB p50 and its phosphorylated form , caspase 3 , and cleaved caspase 3 in the LNCaP human prostate cancer cell line .
	manualset3
98094	11	400966	13	NULL	NULL	0	NULL	LNCaP human prostate cancer cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we evaluated by Western blot the effects in vitro of GHRH and its antagonist JMR-132 on proliferating cell nuclear antigen , tumor suppressor protein p53 , transcription factor NF-kappaB p50 and its phosphorylated form , caspase 3 , and cleaved caspase 3 in the LNCaP human prostate cancer cell line .
	manualset3
98589	9	400966	13	NULL	NULL	0	NULL	 phosphorylated form	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we evaluated by Western blot the effects in vitro of GHRH and its antagonist JMR-132 on proliferating cell nuclear antigen , tumor suppressor protein p53 , transcription factor NF-kappaB p50 and its phosphorylated form , caspase 3 , and cleaved caspase 3 in the LNCaP human prostate cancer cell line .
	manualset3
98095	1	400967	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we evaluated in double-blinded , prospective , randomized manner the dose requirements for remifentanil with thiopental without muscle relaxant administration to obtain clinically acceptable intubation conditions and cardiovascular responses .
	manualset3
98096	2	400967	13	NULL	NULL	NULL	NULL	double-blinded manner 	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , we evaluated in double-blinded , prospective , randomized manner the dose requirements for remifentanil with thiopental without muscle relaxant administration to obtain clinically acceptable intubation conditions and cardiovascular responses .
	manualset3
98097	3	400967	13	NULL	NULL	0	NULL	prospective manner 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we evaluated in double-blinded , prospective , randomized manner the dose requirements for remifentanil with thiopental without muscle relaxant administration to obtain clinically acceptable intubation conditions and cardiovascular responses .
	manualset3
98098	4	400967	13	NULL	NULL	0	NULL	randomized manner	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we evaluated in double-blinded , prospective , randomized manner the dose requirements for remifentanil with thiopental without muscle relaxant administration to obtain clinically acceptable intubation conditions and cardiovascular responses .
	manualset3
98099	5	400967	13	NULL	NULL	0	NULL	dose requirements	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we evaluated in double-blinded , prospective , randomized manner the dose requirements for remifentanil with thiopental without muscle relaxant administration to obtain clinically acceptable intubation conditions and cardiovascular responses .
	manualset3
98100	6	400967	13	NULL	NULL	0	NULL	remifentanil 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we evaluated in double-blinded , prospective , randomized manner the dose requirements for remifentanil with thiopental without muscle relaxant administration to obtain clinically acceptable intubation conditions and cardiovascular responses .
	manualset3
98101	7	400967	13	NULL	NULL	0	NULL	 thiopental	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we evaluated in double-blinded , prospective , randomized manner the dose requirements for remifentanil with thiopental without muscle relaxant administration to obtain clinically acceptable intubation conditions and cardiovascular responses .
	manualset3
98102	8	400967	13	NULL	NULL	0	NULL	muscle relaxant administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we evaluated in double-blinded , prospective , randomized manner the dose requirements for remifentanil with thiopental without muscle relaxant administration to obtain clinically acceptable intubation conditions and cardiovascular responses .
	manualset3
98103	9	400967	13	NULL	NULL	0	NULL	intubation conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we evaluated in double-blinded , prospective , randomized manner the dose requirements for remifentanil with thiopental without muscle relaxant administration to obtain clinically acceptable intubation conditions and cardiovascular responses .
	manualset3
98104	10	400967	13	NULL	NULL	0	NULL	cardiovascular responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we evaluated in double-blinded , prospective , randomized manner the dose requirements for remifentanil with thiopental without muscle relaxant administration to obtain clinically acceptable intubation conditions and cardiovascular responses .
	manualset3
98105	1	400968	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we evaluated the role of TACE in acute inflammation using an inhibitor of the enzyme in a rat model of lung transplantation .
	manualset3
98106	2	400968	13	NULL	NULL	0	NULL	role of TACE	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we evaluated the role of TACE in acute inflammation using an inhibitor of the enzyme in a rat model of lung transplantation .
	manualset3
98107	3	400968	13	NULL	NULL	0	NULL	acute inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we evaluated the role of TACE in acute inflammation using an inhibitor of the enzyme in a rat model of lung transplantation .
	manualset3
98108	4	400968	13	NULL	NULL	0	NULL	inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we evaluated the role of TACE in acute inflammation using an inhibitor of the enzyme in a rat model of lung transplantation .
	manualset3
98109	5	400968	13	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we evaluated the role of TACE in acute inflammation using an inhibitor of the enzyme in a rat model of lung transplantation .
	manualset3
98110	6	400968	13	NULL	NULL	0	NULL	rat model of lung transplantation	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we evaluated the role of TACE in acute inflammation using an inhibitor of the enzyme in a rat model of lung transplantation .
	manualset3
98111	1	400969	13	NULL	NULL	0	NULL	1 1/2 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	11/2 years following resection of an osteosarcoma of the right proximal fibula , pain and roentgenologic lesions of the right tibia at exactly the same level were first of all suspicious of tumor relapse .
	manualset3
98112	2	400969	13	NULL	NULL	0	NULL	resection 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	11/2 years following resection of an osteosarcoma of the right proximal fibula , pain and roentgenologic lesions of the right tibia at exactly the same level were first of all suspicious of tumor relapse .
	manualset3
98113	3	400969	13	NULL	NULL	0	NULL	osteosarcoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	11/2 years following resection of an osteosarcoma of the right proximal fibula , pain and roentgenologic lesions of the right tibia at exactly the same level were first of all suspicious of tumor relapse .
	manualset3
98114	4	400969	13	NULL	NULL	0	NULL	right proximal fibula	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	11/2 years following resection of an osteosarcoma of the right proximal fibula , pain and roentgenologic lesions of the right tibia at exactly the same level were first of all suspicious of tumor relapse .
	manualset3
98115	5	400969	13	NULL	NULL	0	NULL	 pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	11/2 years following resection of an osteosarcoma of the right proximal fibula , pain and roentgenologic lesions of the right tibia at exactly the same level were first of all suspicious of tumor relapse .
	manualset3
98116	6	400969	13	NULL	NULL	0	NULL	roentgenologic lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	11/2 years following resection of an osteosarcoma of the right proximal fibula , pain and roentgenologic lesions of the right tibia at exactly the same level were first of all suspicious of tumor relapse .
	manualset3
98117	7	400969	13	NULL	NULL	0	NULL	right tibia	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	11/2 years following resection of an osteosarcoma of the right proximal fibula , pain and roentgenologic lesions of the right tibia at exactly the same level were first of all suspicious of tumor relapse .
	manualset3
98118	8	400969	13	NULL	NULL	0	NULL	same level	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	11/2 years following resection of an osteosarcoma of the right proximal fibula , pain and roentgenologic lesions of the right tibia at exactly the same level were first of all suspicious of tumor relapse .
	manualset3
98119	9	400969	13	NULL	NULL	0	NULL	tumor relapse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	11/2 years following resection of an osteosarcoma of the right proximal fibula , pain and roentgenologic lesions of the right tibia at exactly the same level were first of all suspicious of tumor relapse .
	manualset3
98120	1	400970	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined secretory response and adaptation of the exocrine pancreas to the administration of free L-homoarginine in normal and bile-pancreatic juice ( BPJ ) - diverted rats .
	manualset3
98121	2	400970	13	NULL	NULL	0	NULL	secretory response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined secretory response and adaptation of the exocrine pancreas to the administration of free L-homoarginine in normal and bile-pancreatic juice ( BPJ ) - diverted rats .
	manualset3
98122	3	400970	13	NULL	NULL	0	NULL	adaptation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined secretory response and adaptation of the exocrine pancreas to the administration of free L-homoarginine in normal and bile-pancreatic juice ( BPJ ) - diverted rats .
	manualset3
98123	4	400970	13	NULL	NULL	0	NULL	exocrine pancreas 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined secretory response and adaptation of the exocrine pancreas to the administration of free L-homoarginine in normal and bile-pancreatic juice ( BPJ ) - diverted rats .
	manualset3
98124	5	400970	13	NULL	NULL	0	NULL	administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined secretory response and adaptation of the exocrine pancreas to the administration of free L-homoarginine in normal and bile-pancreatic juice ( BPJ ) - diverted rats .
	manualset3
98125	6	400970	13	NULL	NULL	0	NULL	L-homoarginine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined secretory response and adaptation of the exocrine pancreas to the administration of free L-homoarginine in normal and bile-pancreatic juice ( BPJ ) - diverted rats .
	manualset3
98126	7	400970	13	NULL	NULL	0	NULL	normal rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined secretory response and adaptation of the exocrine pancreas to the administration of free L-homoarginine in normal and bile-pancreatic juice ( BPJ ) - diverted rats .
	manualset3
98127	8	400970	13	NULL	NULL	0	NULL	bile-pancreatic juice ( BPJ ) - diverted rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined secretory response and adaptation of the exocrine pancreas to the administration of free L-homoarginine in normal and bile-pancreatic juice ( BPJ ) - diverted rats .
	manualset3
98128	1	400971	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined the effect of 15-HPETE on the release of tissue-type plasminogen activator ( t-PA ) and plasminogen activator inhibitor-1 ( PAI-1 ) from cultured human umbilical vein endothelial cells ( HUVEC ) .
	manualset3
98129	2	400971	13	NULL	NULL	0	NULL	effect of 15-HPETE 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined the effect of 15-HPETE on the release of tissue-type plasminogen activator ( t-PA ) and plasminogen activator inhibitor-1 ( PAI-1 ) from cultured human umbilical vein endothelial cells ( HUVEC ) .
	manualset3
98130	3	400971	13	NULL	NULL	0	NULL	release of tissue-type plasminogen activator ( t-PA )	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined the effect of 15-HPETE on the release of tissue-type plasminogen activator ( t-PA ) and plasminogen activator inhibitor-1 ( PAI-1 ) from cultured human umbilical vein endothelial cells ( HUVEC ) .
	manualset3
98131	4	400971	13	NULL	NULL	0	NULL	release of plasminogen activator inhibitor-1 ( PAI-1 )	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined the effect of 15-HPETE on the release of tissue-type plasminogen activator ( t-PA ) and plasminogen activator inhibitor-1 ( PAI-1 ) from cultured human umbilical vein endothelial cells ( HUVEC ) .
	manualset3
98132	5	400971	13	NULL	NULL	0	NULL	human umbilical vein endothelial cells ( HUVEC )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined the effect of 15-HPETE on the release of tissue-type plasminogen activator ( t-PA ) and plasminogen activator inhibitor-1 ( PAI-1 ) from cultured human umbilical vein endothelial cells ( HUVEC ) .
	manualset3
98133	1	400972	13	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined the effects of ex vivo treatment of human cord blood cells with cytokine mixtures and assessed the ability of treated cells to engraft in NOD-scid mice .
	manualset3
98134	2	400972	13	NULL	NULL	0	NULL	effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined the effects of ex vivo treatment of human cord blood cells with cytokine mixtures and assessed the ability of treated cells to engraft in NOD-scid mice .
	manualset3
98135	3	400972	13	NULL	NULL	0	NULL	ex vivo treatment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined the effects of ex vivo treatment of human cord blood cells with cytokine mixtures and assessed the ability of treated cells to engraft in NOD-scid mice .
	manualset3
98136	4	400972	13	NULL	NULL	0	NULL	human cord blood cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined the effects of ex vivo treatment of human cord blood cells with cytokine mixtures and assessed the ability of treated cells to engraft in NOD-scid mice .
	manualset3
98137	5	400972	13	NULL	NULL	0	NULL	cytokine mixtures 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined the effects of ex vivo treatment of human cord blood cells with cytokine mixtures and assessed the ability of treated cells to engraft in NOD-scid mice .
	manualset3
98138	6	400972	13	NULL	NULL	0	NULL	ability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined the effects of ex vivo treatment of human cord blood cells with cytokine mixtures and assessed the ability of treated cells to engraft in NOD-scid mice .
	manualset3
98139	7	400972	13	NULL	NULL	0	NULL	 cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined the effects of ex vivo treatment of human cord blood cells with cytokine mixtures and assessed the ability of treated cells to engraft in NOD-scid mice .
	manualset3
98140	8	400972	13	NULL	NULL	0	NULL	NOD-scid mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined the effects of ex vivo treatment of human cord blood cells with cytokine mixtures and assessed the ability of treated cells to engraft in NOD-scid mice .
	manualset3
98141	1	400973	13	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined the interaction of Ca2 + - CaM with vinflunine , vinblastine , and stable tubule only polypeptide ( STOP ) by using a combination of thermodynamic and mass spectrometric approaches .
	manualset3
98142	2	400973	13	NULL	NULL	0	NULL	interaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined the interaction of Ca2 + - CaM with vinflunine , vinblastine , and stable tubule only polypeptide ( STOP ) by using a combination of thermodynamic and mass spectrometric approaches .
	manualset3
98143	3	400973	13	NULL	NULL	0	NULL	Ca2 + - CaM	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined the interaction of Ca2 + - CaM with vinflunine , vinblastine , and stable tubule only polypeptide ( STOP ) by using a combination of thermodynamic and mass spectrometric approaches .
	manualset3
98144	4	400973	13	NULL	NULL	0	NULL	vinflunine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined the interaction of Ca2 + - CaM with vinflunine , vinblastine , and stable tubule only polypeptide ( STOP ) by using a combination of thermodynamic and mass spectrometric approaches .
	manualset3
98145	5	400973	13	NULL	NULL	0	NULL	vinblastine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined the interaction of Ca2 + - CaM with vinflunine , vinblastine , and stable tubule only polypeptide ( STOP ) by using a combination of thermodynamic and mass spectrometric approaches .
	manualset3
98146	6	400973	13	NULL	NULL	0	NULL	 stable tubule only polypeptide ( STOP )	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined the interaction of Ca2 + - CaM with vinflunine , vinblastine , and stable tubule only polypeptide ( STOP ) by using a combination of thermodynamic and mass spectrometric approaches .
	manualset3
98147	7	400973	13	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined the interaction of Ca2 + - CaM with vinflunine , vinblastine , and stable tubule only polypeptide ( STOP ) by using a combination of thermodynamic and mass spectrometric approaches .
	manualset3
98148	8	400973	13	NULL	NULL	NULL	NULL	 thermodynamic approaches	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , we examined the interaction of Ca2 + - CaM with vinflunine , vinblastine , and stable tubule only polypeptide ( STOP ) by using a combination of thermodynamic and mass spectrometric approaches .
	manualset3
98149	9	400973	13	NULL	NULL	NULL	NULL	mass spectrometric approaches	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , we examined the interaction of Ca2 + - CaM with vinflunine , vinblastine , and stable tubule only polypeptide ( STOP ) by using a combination of thermodynamic and mass spectrometric approaches .
	manualset3
98150	1	400974	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined the role of SP-A in modulating complement receptor-mediated phagocytosis .
	manualset3
98151	2	400974	13	NULL	NULL	NULL	NULL	role 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , we examined the role of SP-A in modulating complement receptor-mediated phagocytosis .
	manualset3
98152	3	400974	13	NULL	NULL	0	NULL	SP-A 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined the role of SP-A in modulating complement receptor-mediated phagocytosis .
	manualset3
98153	4	400974	13	NULL	NULL	NULL	NULL	complement receptor-mediated phagocytosis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , we examined the role of SP-A in modulating complement receptor-mediated phagocytosis .
	manualset3
98154	1	400975	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined whether administration of anti-CD137 mAb can prevent the development of cGVHD after bone marrow transplantation ( BMT ) in mice conditioned with total body irradiation ( TBI ) .
	manualset3
98155	2	400975	13	NULL	NULL	0	NULL	administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined whether administration of anti-CD137 mAb can prevent the development of cGVHD after bone marrow transplantation ( BMT ) in mice conditioned with total body irradiation ( TBI ) .
	manualset3
98156	3	400975	13	NULL	NULL	0	NULL	anti-CD137 mAb	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined whether administration of anti-CD137 mAb can prevent the development of cGVHD after bone marrow transplantation ( BMT ) in mice conditioned with total body irradiation ( TBI ) .
	manualset3
98157	4	400975	13	NULL	NULL	0	NULL	development of cGVHD	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined whether administration of anti-CD137 mAb can prevent the development of cGVHD after bone marrow transplantation ( BMT ) in mice conditioned with total body irradiation ( TBI ) .
	manualset3
98158	5	400975	13	NULL	NULL	0	NULL	bone marrow transplantation ( BMT )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined whether administration of anti-CD137 mAb can prevent the development of cGVHD after bone marrow transplantation ( BMT ) in mice conditioned with total body irradiation ( TBI ) .
	manualset3
98159	6	400975	13	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined whether administration of anti-CD137 mAb can prevent the development of cGVHD after bone marrow transplantation ( BMT ) in mice conditioned with total body irradiation ( TBI ) .
	manualset3
98160	7	400975	13	NULL	NULL	0	NULL	total body irradiation ( TBI )	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we examined whether administration of anti-CD137 mAb can prevent the development of cGVHD after bone marrow transplantation ( BMT ) in mice conditioned with total body irradiation ( TBI ) .
	manualset3
98161	1	400976	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we explore the performance with respect to ML score , running time , and topological accuracy , of FastTree and RAxML on thousands of alignments ( based on both simulated and biological nucleotide datasets ) with up to 27 , 634 sequences .
	manualset3
98162	2	400976	13	NULL	NULL	NULL	NULL	performance	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , we explore the performance with respect to ML score , running time , and topological accuracy , of FastTree and RAxML on thousands of alignments ( based on both simulated and biological nucleotide datasets ) with up to 27 , 634 sequences .
	manualset3
98164	4	400976	13	NULL	NULL	0	NULL	ML score	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we explore the performance with respect to ML score , running time , and topological accuracy , of FastTree and RAxML on thousands of alignments ( based on both simulated and biological nucleotide datasets ) with up to 27 , 634 sequences .
	manualset3
98165	5	400976	13	NULL	NULL	0	NULL	running time 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we explore the performance with respect to ML score , running time , and topological accuracy , of FastTree and RAxML on thousands of alignments ( based on both simulated and biological nucleotide datasets ) with up to 27 , 634 sequences .
	manualset3
98166	6	400976	13	NULL	NULL	0	NULL	topological accuracy	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we explore the performance with respect to ML score , running time , and topological accuracy , of FastTree and RAxML on thousands of alignments ( based on both simulated and biological nucleotide datasets ) with up to 27 , 634 sequences .
	manualset3
98167	7	400976	13	NULL	NULL	0	NULL	FastTree	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we explore the performance with respect to ML score , running time , and topological accuracy , of FastTree and RAxML on thousands of alignments ( based on both simulated and biological nucleotide datasets ) with up to 27 , 634 sequences .
	manualset3
98168	8	400976	13	NULL	NULL	0	NULL	RAxML	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we explore the performance with respect to ML score , running time , and topological accuracy , of FastTree and RAxML on thousands of alignments ( based on both simulated and biological nucleotide datasets ) with up to 27 , 634 sequences .
	manualset3
98169	9	400976	13	NULL	NULL	0	NULL	thousands of alignments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we explore the performance with respect to ML score , running time , and topological accuracy , of FastTree and RAxML on thousands of alignments ( based on both simulated and biological nucleotide datasets ) with up to 27 , 634 sequences .
	manualset3
98170	10	400976	13	NULL	NULL	0	NULL	biological nucleotide datasets 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we explore the performance with respect to ML score , running time , and topological accuracy , of FastTree and RAxML on thousands of alignments ( based on both simulated and biological nucleotide datasets ) with up to 27 , 634 sequences .
	manualset3
98171	12	400976	13	NULL	NULL	NULL	NULL	27 , 634 sequences	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , we explore the performance with respect to ML score , running time , and topological accuracy , of FastTree and RAxML on thousands of alignments ( based on both simulated and biological nucleotide datasets ) with up to 27 , 634 sequences .
	manualset3
98588	11	400976	13	NULL	NULL	0	NULL	simulated datasets	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we explore the performance with respect to ML score , running time , and topological accuracy , of FastTree and RAxML on thousands of alignments ( based on both simulated and biological nucleotide datasets ) with up to 27 , 634 sequences .
	manualset3
98172	1	400977	13	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we have compared the complete nucleotide sequence of the cag PAI in four clinical isolates .
	manualset3
98173	2	400977	13	NULL	NULL	0	NULL	complete nucleotide sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we have compared the complete nucleotide sequence of the cag PAI in four clinical isolates .
	manualset3
98174	3	400977	13	NULL	NULL	0	NULL	cag PAI 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we have compared the complete nucleotide sequence of the cag PAI in four clinical isolates .
	manualset3
98175	4	400977	13	NULL	NULL	0	NULL	four clinical isolates	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we have compared the complete nucleotide sequence of the cag PAI in four clinical isolates .
	manualset3
98176	1	400978	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we have elucidated the temporal and spatial patterns of expression of peroxisome proliferator-activated receptor ( PPAR ) and 9-cis retinoic acid receptor ( RXR ) isoforms in the junctional and labyrinth zones of the developing rat chorioallantoic placenta and in human term placenta .
	manualset3
98177	2	400978	13	NULL	NULL	0	NULL	temporal patterns of expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we have elucidated the temporal and spatial patterns of expression of peroxisome proliferator-activated receptor ( PPAR ) and 9-cis retinoic acid receptor ( RXR ) isoforms in the junctional and labyrinth zones of the developing rat chorioallantoic placenta and in human term placenta .
	manualset3
98178	3	400978	13	NULL	NULL	0	NULL	spatial patterns of expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we have elucidated the temporal and spatial patterns of expression of peroxisome proliferator-activated receptor ( PPAR ) and 9-cis retinoic acid receptor ( RXR ) isoforms in the junctional and labyrinth zones of the developing rat chorioallantoic placenta and in human term placenta .
	manualset3
98179	4	400978	13	NULL	NULL	0	NULL	peroxisome proliferator-activated receptor ( PPAR ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we have elucidated the temporal and spatial patterns of expression of peroxisome proliferator-activated receptor ( PPAR ) and 9-cis retinoic acid receptor ( RXR ) isoforms in the junctional and labyrinth zones of the developing rat chorioallantoic placenta and in human term placenta .
	manualset3
98180	5	400978	13	NULL	NULL	0	NULL	9-cis retinoic acid receptor ( RXR ) isoforms	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we have elucidated the temporal and spatial patterns of expression of peroxisome proliferator-activated receptor ( PPAR ) and 9-cis retinoic acid receptor ( RXR ) isoforms in the junctional and labyrinth zones of the developing rat chorioallantoic placenta and in human term placenta .
	manualset3
98181	6	400978	13	NULL	NULL	0	NULL	junctional zones  	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we have elucidated the temporal and spatial patterns of expression of peroxisome proliferator-activated receptor ( PPAR ) and 9-cis retinoic acid receptor ( RXR ) isoforms in the junctional and labyrinth zones of the developing rat chorioallantoic placenta and in human term placenta .
	manualset3
98182	7	400978	13	NULL	NULL	0	NULL	labyrinth zones	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we have elucidated the temporal and spatial patterns of expression of peroxisome proliferator-activated receptor ( PPAR ) and 9-cis retinoic acid receptor ( RXR ) isoforms in the junctional and labyrinth zones of the developing rat chorioallantoic placenta and in human term placenta .
	manualset3
98183	8	400978	13	NULL	NULL	0	NULL	rat chorioallantoic placenta	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we have elucidated the temporal and spatial patterns of expression of peroxisome proliferator-activated receptor ( PPAR ) and 9-cis retinoic acid receptor ( RXR ) isoforms in the junctional and labyrinth zones of the developing rat chorioallantoic placenta and in human term placenta .
	manualset3
98184	9	400978	13	NULL	NULL	0	NULL	human term placenta	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we have elucidated the temporal and spatial patterns of expression of peroxisome proliferator-activated receptor ( PPAR ) and 9-cis retinoic acid receptor ( RXR ) isoforms in the junctional and labyrinth zones of the developing rat chorioallantoic placenta and in human term placenta .
	manualset3
98185	1	400979	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we have identified a variant of the fyn kinase at 70-72 kDa ( termed p72fyn-R ) that can preferentially associate with the TcR/CD3 complex in certain T cells .
	manualset3
98186	2	400979	13	NULL	NULL	NULL	NULL	variant of the fyn kinase	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , we have identified a variant of the fyn kinase at 70-72 kDa ( termed p72fyn-R ) that can preferentially associate with the TcR/CD3 complex in certain T cells .
	manualset3
98187	5	400979	13	NULL	NULL	NULL	NULL	TcR/CD3 complex 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , we have identified a variant of the fyn kinase at 70-72 kDa ( termed p72fyn-R ) that can preferentially associate with the TcR/CD3 complex in certain T cells .
	manualset3
98188	6	400979	13	NULL	NULL	NULL	NULL	T cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , we have identified a variant of the fyn kinase at 70-72 kDa ( termed p72fyn-R ) that can preferentially associate with the TcR/CD3 complex in certain T cells .
	manualset3
98586	3	400979	13	NULL	NULL	0	NULL	70-72 kDa	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we have identified a variant of the fyn kinase at 70-72 kDa ( termed p72fyn-R ) that can preferentially associate with the TcR/CD3 complex in certain T cells .
	manualset3
98587	4	400979	13	NULL	NULL	0	NULL	p72fyn-R	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we have identified a variant of the fyn kinase at 70-72 kDa ( termed p72fyn-R ) that can preferentially associate with the TcR/CD3 complex in certain T cells .
	manualset3
98189	1	400980	13	NULL	NULL	0	NULL	2 , 2 ' - Anhydro-3 ' - deoxy-5-ethyluridine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , 2 ' - Anhydro-3 ' - deoxy-5-ethyluridine , a new pyrimidine nucleoside analog , has been examined in terms of its binding potency to uridine phosphorylase , and its conformation in solution ( NMR ) was studied .
	manualset3
98190	2	400980	13	NULL	NULL	0	NULL	a new pyrimidine nucleoside analog	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , 2 ' - Anhydro-3 ' - deoxy-5-ethyluridine , a new pyrimidine nucleoside analog , has been examined in terms of its binding potency to uridine phosphorylase , and its conformation in solution ( NMR ) was studied .
	manualset3
98191	3	400980	13	NULL	NULL	NULL	NULL	binding potency	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	2 , 2 ' - Anhydro-3 ' - deoxy-5-ethyluridine , a new pyrimidine nucleoside analog , has been examined in terms of its binding potency to uridine phosphorylase , and its conformation in solution ( NMR ) was studied .
	manualset3
98192	4	400980	13	NULL	NULL	0	NULL	uridine phosphorylase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , 2 ' - Anhydro-3 ' - deoxy-5-ethyluridine , a new pyrimidine nucleoside analog , has been examined in terms of its binding potency to uridine phosphorylase , and its conformation in solution ( NMR ) was studied .
	manualset3
98193	5	400980	13	NULL	NULL	0	NULL	conformation in solution	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , 2 ' - Anhydro-3 ' - deoxy-5-ethyluridine , a new pyrimidine nucleoside analog , has been examined in terms of its binding potency to uridine phosphorylase , and its conformation in solution ( NMR ) was studied .
	manualset3
98194	6	400980	13	NULL	NULL	0	NULL	NMR 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , 2 ' - Anhydro-3 ' - deoxy-5-ethyluridine , a new pyrimidine nucleoside analog , has been examined in terms of its binding potency to uridine phosphorylase , and its conformation in solution ( NMR ) was studied .
	manualset3
98590	1	400981	13	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we have used the yeast two-hybrid approach to screen for proteins that interact with CBS and have identified several components of the sumoylation pathway including Ubc9 , PIAS1 , PIAS3 , Pc2 , and RanBPM .
	manualset3
98591	2	400981	13	NULL	NULL	0	NULL	yeast two-hybrid approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we have used the yeast two-hybrid approach to screen for proteins that interact with CBS and have identified several components of the sumoylation pathway including Ubc9 , PIAS1 , PIAS3 , Pc2 , and RanBPM .
	manualset3
98592	3	400981	13	NULL	NULL	0	NULL	proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we have used the yeast two-hybrid approach to screen for proteins that interact with CBS and have identified several components of the sumoylation pathway including Ubc9 , PIAS1 , PIAS3 , Pc2 , and RanBPM .
	manualset3
98593	4	400981	13	NULL	NULL	0	NULL	CBS 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we have used the yeast two-hybrid approach to screen for proteins that interact with CBS and have identified several components of the sumoylation pathway including Ubc9 , PIAS1 , PIAS3 , Pc2 , and RanBPM .
	manualset3
98594	5	400981	13	NULL	NULL	0	NULL	components 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we have used the yeast two-hybrid approach to screen for proteins that interact with CBS and have identified several components of the sumoylation pathway including Ubc9 , PIAS1 , PIAS3 , Pc2 , and RanBPM .
	manualset3
98595	6	400981	13	NULL	NULL	0	NULL	sumoylation pathway 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we have used the yeast two-hybrid approach to screen for proteins that interact with CBS and have identified several components of the sumoylation pathway including Ubc9 , PIAS1 , PIAS3 , Pc2 , and RanBPM .
	manualset3
98596	7	400981	13	NULL	NULL	0	NULL	Ubc9 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we have used the yeast two-hybrid approach to screen for proteins that interact with CBS and have identified several components of the sumoylation pathway including Ubc9 , PIAS1 , PIAS3 , Pc2 , and RanBPM .
	manualset3
98597	8	400981	13	NULL	NULL	0	NULL	PIAS1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we have used the yeast two-hybrid approach to screen for proteins that interact with CBS and have identified several components of the sumoylation pathway including Ubc9 , PIAS1 , PIAS3 , Pc2 , and RanBPM .
	manualset3
98598	9	400981	13	NULL	NULL	0	NULL	PIAS3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we have used the yeast two-hybrid approach to screen for proteins that interact with CBS and have identified several components of the sumoylation pathway including Ubc9 , PIAS1 , PIAS3 , Pc2 , and RanBPM .
	manualset3
98599	10	400981	13	NULL	NULL	0	NULL	Pc2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we have used the yeast two-hybrid approach to screen for proteins that interact with CBS and have identified several components of the sumoylation pathway including Ubc9 , PIAS1 , PIAS3 , Pc2 , and RanBPM .
	manualset3
98600	11	400981	13	NULL	NULL	0	NULL	RanBPM	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we have used the yeast two-hybrid approach to screen for proteins that interact with CBS and have identified several components of the sumoylation pathway including Ubc9 , PIAS1 , PIAS3 , Pc2 , and RanBPM .
	manualset3
98601	1	400982	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we hypothesized that functional polymorphisms in genes involved in the mitochondrial apoptotic pathway might modulate the apoptotic capacity underlying the muscle loss and contributing to intrafamilial and interfamilial variable phenotypes in LGMD2C ( Limb Girdle Muscular Dystrophy type 2C ) patients sharing the same c. 521delT mutation in SGCG gene .
	manualset3
98602	2	400982	13	NULL	NULL	0	NULL	functional polymorphisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we hypothesized that functional polymorphisms in genes involved in the mitochondrial apoptotic pathway might modulate the apoptotic capacity underlying the muscle loss and contributing to intrafamilial and interfamilial variable phenotypes in LGMD2C ( Limb Girdle Muscular Dystrophy type 2C ) patients sharing the same c. 521delT mutation in SGCG gene .
	manualset3
98603	3	400982	13	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we hypothesized that functional polymorphisms in genes involved in the mitochondrial apoptotic pathway might modulate the apoptotic capacity underlying the muscle loss and contributing to intrafamilial and interfamilial variable phenotypes in LGMD2C ( Limb Girdle Muscular Dystrophy type 2C ) patients sharing the same c. 521delT mutation in SGCG gene .
	manualset3
98604	4	400982	13	NULL	NULL	0	NULL	mitochondrial apoptotic pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we hypothesized that functional polymorphisms in genes involved in the mitochondrial apoptotic pathway might modulate the apoptotic capacity underlying the muscle loss and contributing to intrafamilial and interfamilial variable phenotypes in LGMD2C ( Limb Girdle Muscular Dystrophy type 2C ) patients sharing the same c. 521delT mutation in SGCG gene .
	manualset3
98605	5	400982	13	NULL	NULL	0	NULL	apoptotic capacity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we hypothesized that functional polymorphisms in genes involved in the mitochondrial apoptotic pathway might modulate the apoptotic capacity underlying the muscle loss and contributing to intrafamilial and interfamilial variable phenotypes in LGMD2C ( Limb Girdle Muscular Dystrophy type 2C ) patients sharing the same c. 521delT mutation in SGCG gene .
	manualset3
98606	6	400982	13	NULL	NULL	0	NULL	muscle loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we hypothesized that functional polymorphisms in genes involved in the mitochondrial apoptotic pathway might modulate the apoptotic capacity underlying the muscle loss and contributing to intrafamilial and interfamilial variable phenotypes in LGMD2C ( Limb Girdle Muscular Dystrophy type 2C ) patients sharing the same c. 521delT mutation in SGCG gene .
	manualset3
98607	7	400982	13	NULL	NULL	0	NULL	intrafamilial variable phenotypes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we hypothesized that functional polymorphisms in genes involved in the mitochondrial apoptotic pathway might modulate the apoptotic capacity underlying the muscle loss and contributing to intrafamilial and interfamilial variable phenotypes in LGMD2C ( Limb Girdle Muscular Dystrophy type 2C ) patients sharing the same c. 521delT mutation in SGCG gene .
	manualset3
98608	8	400982	13	NULL	NULL	0	NULL	interfamilial variable phenotypes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we hypothesized that functional polymorphisms in genes involved in the mitochondrial apoptotic pathway might modulate the apoptotic capacity underlying the muscle loss and contributing to intrafamilial and interfamilial variable phenotypes in LGMD2C ( Limb Girdle Muscular Dystrophy type 2C ) patients sharing the same c. 521delT mutation in SGCG gene .
	manualset3
98609	9	400982	13	NULL	NULL	0	NULL	LGMD2C ( Limb Girdle Muscular Dystrophy type 2C ) patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we hypothesized that functional polymorphisms in genes involved in the mitochondrial apoptotic pathway might modulate the apoptotic capacity underlying the muscle loss and contributing to intrafamilial and interfamilial variable phenotypes in LGMD2C ( Limb Girdle Muscular Dystrophy type 2C ) patients sharing the same c. 521delT mutation in SGCG gene .
	manualset3
98610	10	400982	13	NULL	NULL	0	NULL	c. 521delT mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we hypothesized that functional polymorphisms in genes involved in the mitochondrial apoptotic pathway might modulate the apoptotic capacity underlying the muscle loss and contributing to intrafamilial and interfamilial variable phenotypes in LGMD2C ( Limb Girdle Muscular Dystrophy type 2C ) patients sharing the same c. 521delT mutation in SGCG gene .
	manualset3
98611	11	400982	13	NULL	NULL	0	NULL	SGCG gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we hypothesized that functional polymorphisms in genes involved in the mitochondrial apoptotic pathway might modulate the apoptotic capacity underlying the muscle loss and contributing to intrafamilial and interfamilial variable phenotypes in LGMD2C ( Limb Girdle Muscular Dystrophy type 2C ) patients sharing the same c. 521delT mutation in SGCG gene .
	manualset3
98612	1	400983	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we identified evolutionarily conserved molecular components in HSCs by comparing the gene expression profiles of zebrafish , murine , and human HSCs .
	manualset3
98613	2	400983	13	NULL	NULL	0	NULL	molecular components 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we identified evolutionarily conserved molecular components in HSCs by comparing the gene expression profiles of zebrafish , murine , and human HSCs .
	manualset3
98614	3	400983	13	NULL	NULL	0	NULL	HSCs 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we identified evolutionarily conserved molecular components in HSCs by comparing the gene expression profiles of zebrafish , murine , and human HSCs .
	manualset3
98615	4	400983	13	NULL	NULL	NULL	NULL	gene expression profiles	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , we identified evolutionarily conserved molecular components in HSCs by comparing the gene expression profiles of zebrafish , murine , and human HSCs .
	manualset3
98616	5	400983	13	NULL	NULL	0	NULL	zebrafish HSCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we identified evolutionarily conserved molecular components in HSCs by comparing the gene expression profiles of zebrafish , murine , and human HSCs .
	manualset3
98617	6	400983	13	NULL	NULL	0	NULL	murine HSCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we identified evolutionarily conserved molecular components in HSCs by comparing the gene expression profiles of zebrafish , murine , and human HSCs .
	manualset3
98618	7	400983	13	NULL	NULL	0	NULL	human HSCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we identified evolutionarily conserved molecular components in HSCs by comparing the gene expression profiles of zebrafish , murine , and human HSCs .
	manualset3
98619	1	400984	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we identified miR-892a as a negative regulator of CYP1A1 expression .
	manualset3
98620	2	400984	13	NULL	NULL	0	NULL	miR-892a	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we identified miR-892a as a negative regulator of CYP1A1 expression .
	manualset3
98621	3	400984	13	NULL	NULL	0	NULL	negative regulator	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we identified miR-892a as a negative regulator of CYP1A1 expression .
	manualset3
98622	4	400984	13	NULL	NULL	0	NULL	CYP1A1 expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we identified miR-892a as a negative regulator of CYP1A1 expression .
	manualset3
98623	1	400985	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigate the roles of ERK activation in survival , micronucleus formation , and nucleotide excision repair ( NER ) synthesis in arsenite-treated G1-enriched CL3 human non-small-cell lung carcinoma cells .
	manualset3
98624	2	400985	13	NULL	NULL	0	NULL	roles	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigate the roles of ERK activation in survival , micronucleus formation , and nucleotide excision repair ( NER ) synthesis in arsenite-treated G1-enriched CL3 human non-small-cell lung carcinoma cells .
	manualset3
98625	3	400985	13	NULL	NULL	0	NULL	ERK activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigate the roles of ERK activation in survival , micronucleus formation , and nucleotide excision repair ( NER ) synthesis in arsenite-treated G1-enriched CL3 human non-small-cell lung carcinoma cells .
	manualset3
98626	4	400985	13	NULL	NULL	0	NULL	survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigate the roles of ERK activation in survival , micronucleus formation , and nucleotide excision repair ( NER ) synthesis in arsenite-treated G1-enriched CL3 human non-small-cell lung carcinoma cells .
	manualset3
98627	5	400985	13	NULL	NULL	0	NULL	micronucleus formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigate the roles of ERK activation in survival , micronucleus formation , and nucleotide excision repair ( NER ) synthesis in arsenite-treated G1-enriched CL3 human non-small-cell lung carcinoma cells .
	manualset3
98628	6	400985	13	NULL	NULL	0	NULL	nucleotide excision repair ( NER ) synthesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigate the roles of ERK activation in survival , micronucleus formation , and nucleotide excision repair ( NER ) synthesis in arsenite-treated G1-enriched CL3 human non-small-cell lung carcinoma cells .
	manualset3
98629	7	400985	13	NULL	NULL	0	NULL	arsenite-treated G1-enriched CL3 human non-small-cell lung carcinoma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigate the roles of ERK activation in survival , micronucleus formation , and nucleotide excision repair ( NER ) synthesis in arsenite-treated G1-enriched CL3 human non-small-cell lung carcinoma cells .
	manualset3
98630	1	400986	13	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated in vitro anti-inflammatory and pro-aggregative effects of petrocortyne A at non-cytotoxic concentrations on various cellular inflammatory phenomena using the macrophage and monocytic cell lines RAW264 .7 and U937 .
	manualset3
98631	2	400986	13	NULL	NULL	0	NULL	anti-inflammatory effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated in vitro anti-inflammatory and pro-aggregative effects of petrocortyne A at non-cytotoxic concentrations on various cellular inflammatory phenomena using the macrophage and monocytic cell lines RAW264 .7 and U937 .
	manualset3
98632	3	400986	13	NULL	NULL	0	NULL	pro-aggregative effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated in vitro anti-inflammatory and pro-aggregative effects of petrocortyne A at non-cytotoxic concentrations on various cellular inflammatory phenomena using the macrophage and monocytic cell lines RAW264 .7 and U937 .
	manualset3
98633	4	400986	13	NULL	NULL	0	NULL	petrocortyne A	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated in vitro anti-inflammatory and pro-aggregative effects of petrocortyne A at non-cytotoxic concentrations on various cellular inflammatory phenomena using the macrophage and monocytic cell lines RAW264 .7 and U937 .
	manualset3
98634	5	400986	13	NULL	NULL	0	NULL	 non-cytotoxic concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated in vitro anti-inflammatory and pro-aggregative effects of petrocortyne A at non-cytotoxic concentrations on various cellular inflammatory phenomena using the macrophage and monocytic cell lines RAW264 .7 and U937 .
	manualset3
98635	6	400986	13	NULL	NULL	0	NULL	cellular inflammatory phenomena 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated in vitro anti-inflammatory and pro-aggregative effects of petrocortyne A at non-cytotoxic concentrations on various cellular inflammatory phenomena using the macrophage and monocytic cell lines RAW264 .7 and U937 .
	manualset3
98636	7	400986	13	NULL	NULL	0	NULL	macrophage	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated in vitro anti-inflammatory and pro-aggregative effects of petrocortyne A at non-cytotoxic concentrations on various cellular inflammatory phenomena using the macrophage and monocytic cell lines RAW264 .7 and U937 .
	manualset3
98637	8	400986	13	NULL	NULL	0	NULL	monocytic cell line RAW264 .7	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated in vitro anti-inflammatory and pro-aggregative effects of petrocortyne A at non-cytotoxic concentrations on various cellular inflammatory phenomena using the macrophage and monocytic cell lines RAW264 .7 and U937 .
	manualset3
98638	9	400986	13	NULL	NULL	0	NULL	monocytic cell line U937	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated in vitro anti-inflammatory and pro-aggregative effects of petrocortyne A at non-cytotoxic concentrations on various cellular inflammatory phenomena using the macrophage and monocytic cell lines RAW264 .7 and U937 .
	manualset3
98639	1	400987	13	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated the effect of DT-5461a on regional blood flow in various organs including tumor tissue with a radiolabeled tracer-distribution technique using 14C-iodoantipyrine .
	manualset3
98640	2	400987	13	NULL	NULL	0	NULL	effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated the effect of DT-5461a on regional blood flow in various organs including tumor tissue with a radiolabeled tracer-distribution technique using 14C-iodoantipyrine .
	manualset3
98641	3	400987	13	NULL	NULL	0	NULL	DT-5461a	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated the effect of DT-5461a on regional blood flow in various organs including tumor tissue with a radiolabeled tracer-distribution technique using 14C-iodoantipyrine .
	manualset3
98642	4	400987	13	NULL	NULL	0	NULL	regional blood flow 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated the effect of DT-5461a on regional blood flow in various organs including tumor tissue with a radiolabeled tracer-distribution technique using 14C-iodoantipyrine .
	manualset3
98643	5	400987	13	NULL	NULL	0	NULL	various organs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated the effect of DT-5461a on regional blood flow in various organs including tumor tissue with a radiolabeled tracer-distribution technique using 14C-iodoantipyrine .
	manualset3
98644	6	400987	13	NULL	NULL	0	NULL	tumor tissue 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated the effect of DT-5461a on regional blood flow in various organs including tumor tissue with a radiolabeled tracer-distribution technique using 14C-iodoantipyrine .
	manualset3
98645	7	400987	13	NULL	NULL	0	NULL	radiolabeled tracer-distribution technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated the effect of DT-5461a on regional blood flow in various organs including tumor tissue with a radiolabeled tracer-distribution technique using 14C-iodoantipyrine .
	manualset3
98646	8	400987	13	NULL	NULL	0	NULL	14C-iodoantipyrine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated the effect of DT-5461a on regional blood flow in various organs including tumor tissue with a radiolabeled tracer-distribution technique using 14C-iodoantipyrine .
	manualset3
98647	1	400988	13	NULL	NULL	0	NULL	2 , 3-butanediol production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , 3-butanediol production by acetogenic bacteria , an alternative route to chemical synthesis , using industrial waste gas .
	manualset3
98648	2	400988	13	NULL	NULL	0	NULL	acetogenic bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , 3-butanediol production by acetogenic bacteria , an alternative route to chemical synthesis , using industrial waste gas .
	manualset3
98649	3	400988	13	NULL	NULL	0	NULL	alternative route	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , 3-butanediol production by acetogenic bacteria , an alternative route to chemical synthesis , using industrial waste gas .
	manualset3
98650	4	400988	13	NULL	NULL	0	NULL	chemical synthesis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , 3-butanediol production by acetogenic bacteria , an alternative route to chemical synthesis , using industrial waste gas .
	manualset3
98651	5	400988	13	NULL	NULL	0	NULL	industrial waste gas	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , 3-butanediol production by acetogenic bacteria , an alternative route to chemical synthesis , using industrial waste gas .
	manualset3
98652	1	400989	13	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated the effect of combined application of chloropicrin and methyl isothiocyanate ( MITC ) on their transformations and persistence in the environment .
	manualset3
98653	2	400989	13	NULL	NULL	0	NULL	effect of combined application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated the effect of combined application of chloropicrin and methyl isothiocyanate ( MITC ) on their transformations and persistence in the environment .
	manualset3
98654	3	400989	13	NULL	NULL	0	NULL	chloropicrin 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated the effect of combined application of chloropicrin and methyl isothiocyanate ( MITC ) on their transformations and persistence in the environment .
	manualset3
98655	4	400989	13	NULL	NULL	0	NULL	methyl isothiocyanate ( MITC ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated the effect of combined application of chloropicrin and methyl isothiocyanate ( MITC ) on their transformations and persistence in the environment .
	manualset3
98656	5	400989	13	NULL	NULL	0	NULL	transformations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated the effect of combined application of chloropicrin and methyl isothiocyanate ( MITC ) on their transformations and persistence in the environment .
	manualset3
98657	6	400989	13	NULL	NULL	0	NULL	persistence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated the effect of combined application of chloropicrin and methyl isothiocyanate ( MITC ) on their transformations and persistence in the environment .
	manualset3
98658	7	400989	13	NULL	NULL	0	NULL	 environment	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated the effect of combined application of chloropicrin and methyl isothiocyanate ( MITC ) on their transformations and persistence in the environment .
	manualset3
98659	1	400990	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated the effects of brain dopamine depletion , through acute tyrosine and phenylalanine depletion , on plasma prolactin , mood and neuropsychological function in 12 normal subjects .
	manualset3
98660	2	400990	13	NULL	NULL	0	NULL	effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated the effects of brain dopamine depletion , through acute tyrosine and phenylalanine depletion , on plasma prolactin , mood and neuropsychological function in 12 normal subjects .
	manualset3
98661	3	400990	13	NULL	NULL	0	NULL	brain dopamine depletion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated the effects of brain dopamine depletion , through acute tyrosine and phenylalanine depletion , on plasma prolactin , mood and neuropsychological function in 12 normal subjects .
	manualset3
98662	4	400990	13	NULL	NULL	0	NULL	tyrosine depletion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated the effects of brain dopamine depletion , through acute tyrosine and phenylalanine depletion , on plasma prolactin , mood and neuropsychological function in 12 normal subjects .
	manualset3
98663	5	400990	13	NULL	NULL	0	NULL	phenylalanine depletion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated the effects of brain dopamine depletion , through acute tyrosine and phenylalanine depletion , on plasma prolactin , mood and neuropsychological function in 12 normal subjects .
	manualset3
98664	6	400990	13	NULL	NULL	0	NULL	plasma prolactin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated the effects of brain dopamine depletion , through acute tyrosine and phenylalanine depletion , on plasma prolactin , mood and neuropsychological function in 12 normal subjects .
	manualset3
98665	7	400990	13	NULL	NULL	0	NULL	mood	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated the effects of brain dopamine depletion , through acute tyrosine and phenylalanine depletion , on plasma prolactin , mood and neuropsychological function in 12 normal subjects .
	manualset3
98666	8	400990	13	NULL	NULL	0	NULL	 neuropsychological function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated the effects of brain dopamine depletion , through acute tyrosine and phenylalanine depletion , on plasma prolactin , mood and neuropsychological function in 12 normal subjects .
	manualset3
98667	9	400990	13	NULL	NULL	0	NULL	12 normal subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we investigated the effects of brain dopamine depletion , through acute tyrosine and phenylalanine depletion , on plasma prolactin , mood and neuropsychological function in 12 normal subjects .
	manualset3
98668	1	400991	13	NULL	NULL	0	NULL	 study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we isolated seven homeobox genes from the ctenophore Mnemiopsis leidyi and examined their expression through development .
	manualset3
98669	2	400991	13	NULL	NULL	0	NULL	seven homeobox genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we isolated seven homeobox genes from the ctenophore Mnemiopsis leidyi and examined their expression through development .
	manualset3
98670	3	400991	13	NULL	NULL	0	NULL	ctenophore Mnemiopsis leidyi	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we isolated seven homeobox genes from the ctenophore Mnemiopsis leidyi and examined their expression through development .
	manualset3
98671	4	400991	13	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we isolated seven homeobox genes from the ctenophore Mnemiopsis leidyi and examined their expression through development .
	manualset3
98672	5	400991	13	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we isolated seven homeobox genes from the ctenophore Mnemiopsis leidyi and examined their expression through development .
	manualset3
98673	1	400992	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we performed microarray-based expression profiling on liver of zebrafish exposed to 15 parts/million ( ppm ) arsenic ( As ( V ) ) for 8-96 h to identify global transcriptional changes and biological networks involved in arsenic-induced adaptive responses in vivo .
	manualset3
98674	2	400992	13	NULL	NULL	0	NULL	microarray-based expression profiling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we performed microarray-based expression profiling on liver of zebrafish exposed to 15 parts/million ( ppm ) arsenic ( As ( V ) ) for 8-96 h to identify global transcriptional changes and biological networks involved in arsenic-induced adaptive responses in vivo .
	manualset3
98675	3	400992	13	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we performed microarray-based expression profiling on liver of zebrafish exposed to 15 parts/million ( ppm ) arsenic ( As ( V ) ) for 8-96 h to identify global transcriptional changes and biological networks involved in arsenic-induced adaptive responses in vivo .
	manualset3
98676	4	400992	13	NULL	NULL	0	NULL	zebrafish 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we performed microarray-based expression profiling on liver of zebrafish exposed to 15 parts/million ( ppm ) arsenic ( As ( V ) ) for 8-96 h to identify global transcriptional changes and biological networks involved in arsenic-induced adaptive responses in vivo .
	manualset3
98677	5	400992	13	NULL	NULL	0	NULL	15 parts/million ( ppm )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we performed microarray-based expression profiling on liver of zebrafish exposed to 15 parts/million ( ppm ) arsenic ( As ( V ) ) for 8-96 h to identify global transcriptional changes and biological networks involved in arsenic-induced adaptive responses in vivo .
	manualset3
98678	6	400992	13	NULL	NULL	0	NULL	arsenic ( As ( V ) ) 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we performed microarray-based expression profiling on liver of zebrafish exposed to 15 parts/million ( ppm ) arsenic ( As ( V ) ) for 8-96 h to identify global transcriptional changes and biological networks involved in arsenic-induced adaptive responses in vivo .
	manualset3
98679	7	400992	13	NULL	NULL	0	NULL	8-96 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we performed microarray-based expression profiling on liver of zebrafish exposed to 15 parts/million ( ppm ) arsenic ( As ( V ) ) for 8-96 h to identify global transcriptional changes and biological networks involved in arsenic-induced adaptive responses in vivo .
	manualset3
98680	8	400992	13	NULL	NULL	0	NULL	global transcriptional changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we performed microarray-based expression profiling on liver of zebrafish exposed to 15 parts/million ( ppm ) arsenic ( As ( V ) ) for 8-96 h to identify global transcriptional changes and biological networks involved in arsenic-induced adaptive responses in vivo .
	manualset3
98681	9	400992	13	NULL	NULL	0	NULL	biological networks	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we performed microarray-based expression profiling on liver of zebrafish exposed to 15 parts/million ( ppm ) arsenic ( As ( V ) ) for 8-96 h to identify global transcriptional changes and biological networks involved in arsenic-induced adaptive responses in vivo .
	manualset3
98682	10	400992	13	NULL	NULL	0	NULL	arsenic-induced adaptive responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we performed microarray-based expression profiling on liver of zebrafish exposed to 15 parts/million ( ppm ) arsenic ( As ( V ) ) for 8-96 h to identify global transcriptional changes and biological networks involved in arsenic-induced adaptive responses in vivo .
	manualset3
98683	1	400993	13	NULL	NULL	0	NULL	 study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we prepared diblock copolymers of poly ( epsilon-caprolactone ) ( PCL ) and poly ( ethylene glycol ) ( PEG ) by aluminum alkoxide catalysts .
	manualset3
98684	2	400993	13	NULL	NULL	0	NULL	copolymers of poly ( epsilon-caprolactone ) ( PCL )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we prepared diblock copolymers of poly ( epsilon-caprolactone ) ( PCL ) and poly ( ethylene glycol ) ( PEG ) by aluminum alkoxide catalysts .
	manualset3
98685	3	400993	13	NULL	NULL	0	NULL	poly ( ethylene glycol ) ( PEG )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we prepared diblock copolymers of poly ( epsilon-caprolactone ) ( PCL ) and poly ( ethylene glycol ) ( PEG ) by aluminum alkoxide catalysts .
	manualset3
98686	4	400993	13	NULL	NULL	0	NULL	 aluminum alkoxide catalysts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we prepared diblock copolymers of poly ( epsilon-caprolactone ) ( PCL ) and poly ( ethylene glycol ) ( PEG ) by aluminum alkoxide catalysts .
	manualset3
98687	1	400994	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we present the clinical and pathologic features of HPS cases who underwent liver transplantation ( LT ) .
	manualset3
98688	2	400994	13	NULL	NULL	0	NULL	clinical features	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we present the clinical and pathologic features of HPS cases who underwent liver transplantation ( LT ) .
	manualset3
98689	3	400994	13	NULL	NULL	0	NULL	pathologic features	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we present the clinical and pathologic features of HPS cases who underwent liver transplantation ( LT ) .
	manualset3
98690	4	400994	13	NULL	NULL	0	NULL	HPS cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we present the clinical and pathologic features of HPS cases who underwent liver transplantation ( LT ) .
	manualset3
98691	5	400994	13	NULL	NULL	0	NULL	liver transplantation ( LT )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we present the clinical and pathologic features of HPS cases who underwent liver transplantation ( LT ) .
	manualset3
98692	1	400995	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we report that allelic exclusion is not regulated by competition between distinct alpha-chains for a single beta-chain , as proposed by the dueling alpha-chain model , nor by limiting CD3 zeta-chain in mature TCR ( high ) thymocytes .
	manualset3
98693	2	400995	13	NULL	NULL	0	NULL	allelic exclusion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we report that allelic exclusion is not regulated by competition between distinct alpha-chains for a single beta-chain , as proposed by the dueling alpha-chain model , nor by limiting CD3 zeta-chain in mature TCR ( high ) thymocytes .
	manualset3
98694	3	400995	13	NULL	NULL	0	NULL	competition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we report that allelic exclusion is not regulated by competition between distinct alpha-chains for a single beta-chain , as proposed by the dueling alpha-chain model , nor by limiting CD3 zeta-chain in mature TCR ( high ) thymocytes .
	manualset3
98695	4	400995	13	NULL	NULL	0	NULL	alpha-chains	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we report that allelic exclusion is not regulated by competition between distinct alpha-chains for a single beta-chain , as proposed by the dueling alpha-chain model , nor by limiting CD3 zeta-chain in mature TCR ( high ) thymocytes .
	manualset3
98696	5	400995	13	NULL	NULL	0	NULL	beta-chain 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we report that allelic exclusion is not regulated by competition between distinct alpha-chains for a single beta-chain , as proposed by the dueling alpha-chain model , nor by limiting CD3 zeta-chain in mature TCR ( high ) thymocytes .
	manualset3
98697	6	400995	13	NULL	NULL	0	NULL	alpha-chain model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we report that allelic exclusion is not regulated by competition between distinct alpha-chains for a single beta-chain , as proposed by the dueling alpha-chain model , nor by limiting CD3 zeta-chain in mature TCR ( high ) thymocytes .
	manualset3
98698	7	400995	13	NULL	NULL	0	NULL	CD3 zeta-chain	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we report that allelic exclusion is not regulated by competition between distinct alpha-chains for a single beta-chain , as proposed by the dueling alpha-chain model , nor by limiting CD3 zeta-chain in mature TCR ( high ) thymocytes .
	manualset3
98699	8	400995	13	NULL	NULL	0	NULL	 mature TCR ( high ) thymocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we report that allelic exclusion is not regulated by competition between distinct alpha-chains for a single beta-chain , as proposed by the dueling alpha-chain model , nor by limiting CD3 zeta-chain in mature TCR ( high ) thymocytes .
	manualset3
98700	1	400996	13	NULL	NULL	0	NULL	2 , 4-Diamino-5 - ( 5 ' - ( 5-carboxypentyl ) -2 ' - methoxybenzyl ) pyrimidine ( 6 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , 4-Diamino-5 - ( 5 ' - ( 5-carboxypentyl ) -2 ' - methoxybenzyl ) pyrimidine ( 6 ) had a selectivity index of 490 against Tg DHFR and was 320 times more potent than TMP .
	manualset3
98701	2	400996	13	NULL	NULL	0	NULL	selectivity index of 490	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , 4-Diamino-5 - ( 5 ' - ( 5-carboxypentyl ) -2 ' - methoxybenzyl ) pyrimidine ( 6 ) had a selectivity index of 490 against Tg DHFR and was 320 times more potent than TMP .
	manualset3
98702	3	400996	13	NULL	NULL	0	NULL	Tg DHFR 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , 4-Diamino-5 - ( 5 ' - ( 5-carboxypentyl ) -2 ' - methoxybenzyl ) pyrimidine ( 6 ) had a selectivity index of 490 against Tg DHFR and was 320 times more potent than TMP .
	manualset3
98703	4	400996	13	NULL	NULL	NULL	NULL	320 times 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	2 , 4-Diamino-5 - ( 5 ' - ( 5-carboxypentyl ) -2 ' - methoxybenzyl ) pyrimidine ( 6 ) had a selectivity index of 490 against Tg DHFR and was 320 times more potent than TMP .
	manualset3
98704	5	400996	13	NULL	NULL	0	NULL	TMP	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , 4-Diamino-5 - ( 5 ' - ( 5-carboxypentyl ) -2 ' - methoxybenzyl ) pyrimidine ( 6 ) had a selectivity index of 490 against Tg DHFR and was 320 times more potent than TMP .
	manualset3
98705	1	400997	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we show COUP-TFII expression in human umbilical vein endothelial cells ( HUVECs ) and human coronary artery endothelial cells .
	manualset3
98706	2	400997	13	NULL	NULL	0	NULL	COUP-TFII expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we show COUP-TFII expression in human umbilical vein endothelial cells ( HUVECs ) and human coronary artery endothelial cells .
	manualset3
98707	3	400997	13	NULL	NULL	0	NULL	human umbilical vein endothelial cells ( HUVECs )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we show COUP-TFII expression in human umbilical vein endothelial cells ( HUVECs ) and human coronary artery endothelial cells .
	manualset3
98708	4	400997	13	NULL	NULL	0	NULL	human coronary artery endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we show COUP-TFII expression in human umbilical vein endothelial cells ( HUVECs ) and human coronary artery endothelial cells .
	manualset3
98709	1	400998	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we show that Gpr126 is essential for myelination and other aspects of peripheral nerve development in mammals .
	manualset3
98710	2	400998	13	NULL	NULL	0	NULL	Gpr126 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we show that Gpr126 is essential for myelination and other aspects of peripheral nerve development in mammals .
	manualset3
98711	3	400998	13	NULL	NULL	0	NULL	myelination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we show that Gpr126 is essential for myelination and other aspects of peripheral nerve development in mammals .
	manualset3
98712	4	400998	13	NULL	NULL	0	NULL	other aspects 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we show that Gpr126 is essential for myelination and other aspects of peripheral nerve development in mammals .
	manualset3
98713	5	400998	13	NULL	NULL	0	NULL	peripheral nerve development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we show that Gpr126 is essential for myelination and other aspects of peripheral nerve development in mammals .
	manualset3
98714	6	400998	13	NULL	NULL	0	NULL	 mammals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we show that Gpr126 is essential for myelination and other aspects of peripheral nerve development in mammals .
	manualset3
98715	1	400999	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we show that failure of endosperm cellularization in fertilization independent seed 2 ( fis2 ) and endosperm defective 1 ( ede1 ) Arabidopsis mutants correlates with impaired embryo development .
	manualset3
98716	2	400999	13	NULL	NULL	0	NULL	failure	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we show that failure of endosperm cellularization in fertilization independent seed 2 ( fis2 ) and endosperm defective 1 ( ede1 ) Arabidopsis mutants correlates with impaired embryo development .
	manualset3
98717	3	400999	13	NULL	NULL	0	NULL	endosperm cellularization 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we show that failure of endosperm cellularization in fertilization independent seed 2 ( fis2 ) and endosperm defective 1 ( ede1 ) Arabidopsis mutants correlates with impaired embryo development .
	manualset3
98718	4	400999	13	NULL	NULL	0	NULL	fertilization independent seed 2 ( fis2 ) 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we show that failure of endosperm cellularization in fertilization independent seed 2 ( fis2 ) and endosperm defective 1 ( ede1 ) Arabidopsis mutants correlates with impaired embryo development .
	manualset3
98719	5	400999	13	NULL	NULL	0	NULL	endosperm defective 1 ( ede1 ) Arabidopsis mutants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we show that failure of endosperm cellularization in fertilization independent seed 2 ( fis2 ) and endosperm defective 1 ( ede1 ) Arabidopsis mutants correlates with impaired embryo development .
	manualset3
98720	6	400999	13	NULL	NULL	0	NULL	embryo development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we show that failure of endosperm cellularization in fertilization independent seed 2 ( fis2 ) and endosperm defective 1 ( ede1 ) Arabidopsis mutants correlates with impaired embryo development .
	manualset3
98721	1	401000	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we show that mating-type II cells accumulate near the site where gamone 1 secreted by mating-type I cells is present at a high concentration .
	manualset3
98722	2	401000	13	NULL	NULL	0	NULL	mating-type II cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we show that mating-type II cells accumulate near the site where gamone 1 secreted by mating-type I cells is present at a high concentration .
	manualset3
98723	3	401000	13	NULL	NULL	0	NULL	site 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we show that mating-type II cells accumulate near the site where gamone 1 secreted by mating-type I cells is present at a high concentration .
	manualset3
98724	4	401000	13	NULL	NULL	NULL	NULL	gamone 1	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , we show that mating-type II cells accumulate near the site where gamone 1 secreted by mating-type I cells is present at a high concentration .
	manualset3
98725	5	401000	13	NULL	NULL	0	NULL	mating-type I cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we show that mating-type II cells accumulate near the site where gamone 1 secreted by mating-type I cells is present at a high concentration .
	manualset3
98726	6	401000	13	NULL	NULL	0	NULL	high concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we show that mating-type II cells accumulate near the site where gamone 1 secreted by mating-type I cells is present at a high concentration .
	manualset3
98727	1	401001	13	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we show that the IgG-Ag retroviral constructs , expressing myelin basic protein ( MBP ) or glutamic acid decarboxylase in B cells , can be used for the treatment of murine models for multiple sclerosis and diabetes .
	manualset3
98728	2	401001	13	NULL	NULL	0	NULL	IgG-Ag retroviral constructs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we show that the IgG-Ag retroviral constructs , expressing myelin basic protein ( MBP ) or glutamic acid decarboxylase in B cells , can be used for the treatment of murine models for multiple sclerosis and diabetes .
	manualset3
98729	3	401001	13	NULL	NULL	0	NULL	myelin basic protein ( MBP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we show that the IgG-Ag retroviral constructs , expressing myelin basic protein ( MBP ) or glutamic acid decarboxylase in B cells , can be used for the treatment of murine models for multiple sclerosis and diabetes .
	manualset3
98730	4	401001	13	NULL	NULL	0	NULL	glutamic acid decarboxylase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we show that the IgG-Ag retroviral constructs , expressing myelin basic protein ( MBP ) or glutamic acid decarboxylase in B cells , can be used for the treatment of murine models for multiple sclerosis and diabetes .
	manualset3
98731	5	401001	13	NULL	NULL	0	NULL	B cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we show that the IgG-Ag retroviral constructs , expressing myelin basic protein ( MBP ) or glutamic acid decarboxylase in B cells , can be used for the treatment of murine models for multiple sclerosis and diabetes .
	manualset3
98732	6	401001	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we show that the IgG-Ag retroviral constructs , expressing myelin basic protein ( MBP ) or glutamic acid decarboxylase in B cells , can be used for the treatment of murine models for multiple sclerosis and diabetes .
	manualset3
98733	7	401001	13	NULL	NULL	0	NULL	murine models for multiple sclerosis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we show that the IgG-Ag retroviral constructs , expressing myelin basic protein ( MBP ) or glutamic acid decarboxylase in B cells , can be used for the treatment of murine models for multiple sclerosis and diabetes .
	manualset3
98734	8	401001	13	NULL	NULL	0	NULL	murine models for diabetes	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we show that the IgG-Ag retroviral constructs , expressing myelin basic protein ( MBP ) or glutamic acid decarboxylase in B cells , can be used for the treatment of murine models for multiple sclerosis and diabetes .
	manualset3
98735	1	401002	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we showed that immature viable DC have the ability to uptake apoptotic DC as well as necrotic DC without it being recognized as an inflammatory event by immature viable DC .
	manualset3
98736	2	401002	13	NULL	NULL	0	NULL	immature viable DC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we showed that immature viable DC have the ability to uptake apoptotic DC as well as necrotic DC without it being recognized as an inflammatory event by immature viable DC .
	manualset3
98737	3	401002	13	NULL	NULL	0	NULL	ability 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we showed that immature viable DC have the ability to uptake apoptotic DC as well as necrotic DC without it being recognized as an inflammatory event by immature viable DC .
	manualset3
98738	4	401002	13	NULL	NULL	0	NULL	apoptotic DC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we showed that immature viable DC have the ability to uptake apoptotic DC as well as necrotic DC without it being recognized as an inflammatory event by immature viable DC .
	manualset3
98739	5	401002	13	NULL	NULL	0	NULL	necrotic DC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we showed that immature viable DC have the ability to uptake apoptotic DC as well as necrotic DC without it being recognized as an inflammatory event by immature viable DC .
	manualset3
98740	6	401002	13	NULL	NULL	0	NULL	 inflammatory event	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we showed that immature viable DC have the ability to uptake apoptotic DC as well as necrotic DC without it being recognized as an inflammatory event by immature viable DC .
	manualset3
98741	7	401002	13	NULL	NULL	0	NULL	 immature viable DC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we showed that immature viable DC have the ability to uptake apoptotic DC as well as necrotic DC without it being recognized as an inflammatory event by immature viable DC .
	manualset3
98742	1	401003	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we tested whether the braconid Asobara tabida , a parasitoid of Drosophila larvae , retains information gleaned on patch quality in the memory and adjusts its foraging behavior accordingly .
	manualset3
98743	2	401003	13	NULL	NULL	0	NULL	braconid Asobara tabida	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we tested whether the braconid Asobara tabida , a parasitoid of Drosophila larvae , retains information gleaned on patch quality in the memory and adjusts its foraging behavior accordingly .
	manualset3
98744	3	401003	13	NULL	NULL	0	NULL	parasitoid of Drosophila larvae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we tested whether the braconid Asobara tabida , a parasitoid of Drosophila larvae , retains information gleaned on patch quality in the memory and adjusts its foraging behavior accordingly .
	manualset3
98745	4	401003	13	NULL	NULL	0	NULL	information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we tested whether the braconid Asobara tabida , a parasitoid of Drosophila larvae , retains information gleaned on patch quality in the memory and adjusts its foraging behavior accordingly .
	manualset3
98746	5	401003	13	NULL	NULL	0	NULL	patch quality	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we tested whether the braconid Asobara tabida , a parasitoid of Drosophila larvae , retains information gleaned on patch quality in the memory and adjusts its foraging behavior accordingly .
	manualset3
98747	6	401003	13	NULL	NULL	0	NULL	memory	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we tested whether the braconid Asobara tabida , a parasitoid of Drosophila larvae , retains information gleaned on patch quality in the memory and adjusts its foraging behavior accordingly .
	manualset3
98748	7	401003	13	NULL	NULL	0	NULL	behavior 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we tested whether the braconid Asobara tabida , a parasitoid of Drosophila larvae , retains information gleaned on patch quality in the memory and adjusts its foraging behavior accordingly .
	manualset3
98749	1	401004	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we used small interfering RNA directed against either Rac1 or Rac3 to reduce their expression specifically .
	manualset3
98750	2	401004	13	NULL	NULL	0	NULL	small interfering RNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we used small interfering RNA directed against either Rac1 or Rac3 to reduce their expression specifically .
	manualset3
98751	3	401004	13	NULL	NULL	0	NULL	Rac1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we used small interfering RNA directed against either Rac1 or Rac3 to reduce their expression specifically .
	manualset3
98752	4	401004	13	NULL	NULL	0	NULL	 Rac3	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we used small interfering RNA directed against either Rac1 or Rac3 to reduce their expression specifically .
	manualset3
98753	5	401004	13	NULL	NULL	0	NULL	 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we used small interfering RNA directed against either Rac1 or Rac3 to reduce their expression specifically .
	manualset3
98754	1	401005	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study IDH1 and IDH2 mutations were detected in a series of 203 gliomas .
	manualset3
98755	2	401005	13	NULL	NULL	0	NULL	 IDH1 mutations  	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study IDH1 and IDH2 mutations were detected in a series of 203 gliomas .
	manualset3
98756	3	401005	13	NULL	NULL	0	NULL	IDH2 mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study IDH1 and IDH2 mutations were detected in a series of 203 gliomas .
	manualset3
98757	4	401005	13	NULL	NULL	0	NULL	series of 203 gliomas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study IDH1 and IDH2 mutations were detected in a series of 203 gliomas .
	manualset3
98758	1	401006	13	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study of the unique stability of the marsupial acrosome , experiments were carried out on the acrosomes of spermatozoa of the tammar wallaby ( Macropus eugenii ) , common brushtail possum ( Trichosurus vulpecula ) and gray short-tailed opossum ( Monodelphis domestica ) .
	manualset3
98759	2	401006	13	NULL	NULL	0	NULL	unique stability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study of the unique stability of the marsupial acrosome , experiments were carried out on the acrosomes of spermatozoa of the tammar wallaby ( Macropus eugenii ) , common brushtail possum ( Trichosurus vulpecula ) and gray short-tailed opossum ( Monodelphis domestica ) .
	manualset3
98760	3	401006	13	NULL	NULL	0	NULL	marsupial acrosome 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study of the unique stability of the marsupial acrosome , experiments were carried out on the acrosomes of spermatozoa of the tammar wallaby ( Macropus eugenii ) , common brushtail possum ( Trichosurus vulpecula ) and gray short-tailed opossum ( Monodelphis domestica ) .
	manualset3
98761	4	401006	13	NULL	NULL	0	NULL	experiments 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study of the unique stability of the marsupial acrosome , experiments were carried out on the acrosomes of spermatozoa of the tammar wallaby ( Macropus eugenii ) , common brushtail possum ( Trichosurus vulpecula ) and gray short-tailed opossum ( Monodelphis domestica ) .
	manualset3
98762	5	401006	13	NULL	NULL	0	NULL	acrosomes of spermatozoa	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study of the unique stability of the marsupial acrosome , experiments were carried out on the acrosomes of spermatozoa of the tammar wallaby ( Macropus eugenii ) , common brushtail possum ( Trichosurus vulpecula ) and gray short-tailed opossum ( Monodelphis domestica ) .
	manualset3
98763	6	401006	13	NULL	NULL	0	NULL	tammar wallaby ( Macropus eugenii )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study of the unique stability of the marsupial acrosome , experiments were carried out on the acrosomes of spermatozoa of the tammar wallaby ( Macropus eugenii ) , common brushtail possum ( Trichosurus vulpecula ) and gray short-tailed opossum ( Monodelphis domestica ) .
	manualset3
98764	7	401006	13	NULL	NULL	0	NULL	common brushtail possum ( Trichosurus vulpecula ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study of the unique stability of the marsupial acrosome , experiments were carried out on the acrosomes of spermatozoa of the tammar wallaby ( Macropus eugenii ) , common brushtail possum ( Trichosurus vulpecula ) and gray short-tailed opossum ( Monodelphis domestica ) .
	manualset3
98765	8	401006	13	NULL	NULL	0	NULL	gray short-tailed opossum ( Monodelphis domestica )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study of the unique stability of the marsupial acrosome , experiments were carried out on the acrosomes of spermatozoa of the tammar wallaby ( Macropus eugenii ) , common brushtail possum ( Trichosurus vulpecula ) and gray short-tailed opossum ( Monodelphis domestica ) .
	manualset3
98766	1	401007	13	NULL	NULL	0	NULL	 study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study the aim was to compare the performances of vaginal , cervical and urinary specimens in a population of young women with sparse symptoms .
	manualset3
98767	2	401007	13	NULL	NULL	0	NULL	 aim	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study the aim was to compare the performances of vaginal , cervical and urinary specimens in a population of young women with sparse symptoms .
	manualset3
98768	3	401007	13	NULL	NULL	0	NULL	performances	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study the aim was to compare the performances of vaginal , cervical and urinary specimens in a population of young women with sparse symptoms .
	manualset3
98769	4	401007	13	NULL	NULL	0	NULL	vaginal specimens	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study the aim was to compare the performances of vaginal , cervical and urinary specimens in a population of young women with sparse symptoms .
	manualset3
98770	5	401007	13	NULL	NULL	0	NULL	cervical specimens 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study the aim was to compare the performances of vaginal , cervical and urinary specimens in a population of young women with sparse symptoms .
	manualset3
98771	6	401007	13	NULL	NULL	0	NULL	urinary specimens	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study the aim was to compare the performances of vaginal , cervical and urinary specimens in a population of young women with sparse symptoms .
	manualset3
98772	7	401007	13	NULL	NULL	0	NULL	 population 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study the aim was to compare the performances of vaginal , cervical and urinary specimens in a population of young women with sparse symptoms .
	manualset3
98773	8	401007	13	NULL	NULL	0	NULL	young women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study the aim was to compare the performances of vaginal , cervical and urinary specimens in a population of young women with sparse symptoms .
	manualset3
98774	9	401007	13	NULL	NULL	0	NULL	sparse symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study the aim was to compare the performances of vaginal , cervical and urinary specimens in a population of young women with sparse symptoms .
	manualset3
98775	1	401008	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study the effect on hospital charges of back transports was examined by comparing the charges for care in community hospitals with what these charges would have been in a tertiary care center .
	manualset3
98776	2	401008	13	NULL	NULL	0	NULL	effect on hospital charges	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study the effect on hospital charges of back transports was examined by comparing the charges for care in community hospitals with what these charges would have been in a tertiary care center .
	manualset3
98777	3	401008	13	NULL	NULL	0	NULL	back transports	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study the effect on hospital charges of back transports was examined by comparing the charges for care in community hospitals with what these charges would have been in a tertiary care center .
	manualset3
98778	4	401008	13	NULL	NULL	0	NULL	charges for care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study the effect on hospital charges of back transports was examined by comparing the charges for care in community hospitals with what these charges would have been in a tertiary care center .
	manualset3
98779	5	401008	13	NULL	NULL	0	NULL	community hospitals	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study the effect on hospital charges of back transports was examined by comparing the charges for care in community hospitals with what these charges would have been in a tertiary care center .
	manualset3
98780	6	401008	13	NULL	NULL	0	NULL	charges 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study the effect on hospital charges of back transports was examined by comparing the charges for care in community hospitals with what these charges would have been in a tertiary care center .
	manualset3
98781	7	401008	13	NULL	NULL	0	NULL	tertiary care center	Facility							tertiary care center					NULL		0	NULL	NULL	NULL	NULL	NULL	In this study the effect on hospital charges of back transports was examined by comparing the charges for care in community hospitals with what these charges would have been in a tertiary care center .
	manualset3
98782	1	401009	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we have developed a simple and rapid procedure that combines a Chelex-based DNA extraction procedure with LAMP to rapidly detect the presence of Mediterranean fruit fly DNA and discriminate it from other species , by using material from different stages of development .
	manualset3
98783	2	401009	13	NULL	NULL	0	NULL	 simple procedure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we have developed a simple and rapid procedure that combines a Chelex-based DNA extraction procedure with LAMP to rapidly detect the presence of Mediterranean fruit fly DNA and discriminate it from other species , by using material from different stages of development .
	manualset3
98784	3	401009	13	NULL	NULL	0	NULL	rapid procedure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we have developed a simple and rapid procedure that combines a Chelex-based DNA extraction procedure with LAMP to rapidly detect the presence of Mediterranean fruit fly DNA and discriminate it from other species , by using material from different stages of development .
	manualset3
98785	4	401009	13	NULL	NULL	0	NULL	Chelex-based DNA extraction procedure 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we have developed a simple and rapid procedure that combines a Chelex-based DNA extraction procedure with LAMP to rapidly detect the presence of Mediterranean fruit fly DNA and discriminate it from other species , by using material from different stages of development .
	manualset3
98786	5	401009	13	NULL	NULL	0	NULL	LAMP 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we have developed a simple and rapid procedure that combines a Chelex-based DNA extraction procedure with LAMP to rapidly detect the presence of Mediterranean fruit fly DNA and discriminate it from other species , by using material from different stages of development .
	manualset3
98787	6	401009	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we have developed a simple and rapid procedure that combines a Chelex-based DNA extraction procedure with LAMP to rapidly detect the presence of Mediterranean fruit fly DNA and discriminate it from other species , by using material from different stages of development .
	manualset3
98788	7	401009	13	NULL	NULL	0	NULL	 Mediterranean fruit fly DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we have developed a simple and rapid procedure that combines a Chelex-based DNA extraction procedure with LAMP to rapidly detect the presence of Mediterranean fruit fly DNA and discriminate it from other species , by using material from different stages of development .
	manualset3
98789	8	401009	13	NULL	NULL	0	NULL	species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we have developed a simple and rapid procedure that combines a Chelex-based DNA extraction procedure with LAMP to rapidly detect the presence of Mediterranean fruit fly DNA and discriminate it from other species , by using material from different stages of development .
	manualset3
98790	9	401009	13	NULL	NULL	0	NULL	material	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we have developed a simple and rapid procedure that combines a Chelex-based DNA extraction procedure with LAMP to rapidly detect the presence of Mediterranean fruit fly DNA and discriminate it from other species , by using material from different stages of development .
	manualset3
98791	10	401009	13	NULL	NULL	0	NULL	different stages of development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we have developed a simple and rapid procedure that combines a Chelex-based DNA extraction procedure with LAMP to rapidly detect the presence of Mediterranean fruit fly DNA and discriminate it from other species , by using material from different stages of development .
	manualset3
98792	1	401010	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we have elucidated the contribution of the hydrophobic effect to multivalent cation - and cationic lipid-DNA binding and DNA collapse by studying the thermodynamics of cobalt hexammine - , spermine - , and lipospermine-plasmid DNA binding at different temperatures .
	manualset3
98793	2	401010	13	NULL	NULL	0	NULL	contribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we have elucidated the contribution of the hydrophobic effect to multivalent cation - and cationic lipid-DNA binding and DNA collapse by studying the thermodynamics of cobalt hexammine - , spermine - , and lipospermine-plasmid DNA binding at different temperatures .
	manualset3
98794	3	401010	13	NULL	NULL	0	NULL	hydrophobic effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we have elucidated the contribution of the hydrophobic effect to multivalent cation - and cationic lipid-DNA binding and DNA collapse by studying the thermodynamics of cobalt hexammine - , spermine - , and lipospermine-plasmid DNA binding at different temperatures .
	manualset3
98795	4	401010	13	NULL	NULL	0	NULL	multivalent cation-DNA binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we have elucidated the contribution of the hydrophobic effect to multivalent cation - and cationic lipid-DNA binding and DNA collapse by studying the thermodynamics of cobalt hexammine - , spermine - , and lipospermine-plasmid DNA binding at different temperatures .
	manualset3
98796	5	401010	13	NULL	NULL	0	NULL	cationic lipid-DNA binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we have elucidated the contribution of the hydrophobic effect to multivalent cation - and cationic lipid-DNA binding and DNA collapse by studying the thermodynamics of cobalt hexammine - , spermine - , and lipospermine-plasmid DNA binding at different temperatures .
	manualset3
98797	6	401010	13	NULL	NULL	0	NULL	DNA collapse	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we have elucidated the contribution of the hydrophobic effect to multivalent cation - and cationic lipid-DNA binding and DNA collapse by studying the thermodynamics of cobalt hexammine - , spermine - , and lipospermine-plasmid DNA binding at different temperatures .
	manualset3
98798	7	401010	13	NULL	NULL	0	NULL	thermodynamics of cobalt 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we have elucidated the contribution of the hydrophobic effect to multivalent cation - and cationic lipid-DNA binding and DNA collapse by studying the thermodynamics of cobalt hexammine - , spermine - , and lipospermine-plasmid DNA binding at different temperatures .
	manualset3
98799	8	401010	13	NULL	NULL	0	NULL	hexammine - plasmid DNA binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we have elucidated the contribution of the hydrophobic effect to multivalent cation - and cationic lipid-DNA binding and DNA collapse by studying the thermodynamics of cobalt hexammine - , spermine - , and lipospermine-plasmid DNA binding at different temperatures .
	manualset3
98800	9	401010	13	NULL	NULL	0	NULL	spermine -plasmid DNA binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we have elucidated the contribution of the hydrophobic effect to multivalent cation - and cationic lipid-DNA binding and DNA collapse by studying the thermodynamics of cobalt hexammine - , spermine - , and lipospermine-plasmid DNA binding at different temperatures .
	manualset3
98801	10	401010	13	NULL	NULL	0	NULL	lipospermine-plasmid DNA binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we have elucidated the contribution of the hydrophobic effect to multivalent cation - and cationic lipid-DNA binding and DNA collapse by studying the thermodynamics of cobalt hexammine - , spermine - , and lipospermine-plasmid DNA binding at different temperatures .
	manualset3
98802	11	401010	13	NULL	NULL	0	NULL	different temperatures	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we have elucidated the contribution of the hydrophobic effect to multivalent cation - and cationic lipid-DNA binding and DNA collapse by studying the thermodynamics of cobalt hexammine - , spermine - , and lipospermine-plasmid DNA binding at different temperatures .
	manualset3
98905	1	401011	13	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigate the roles of the cytohesin ADP-ribosylation factor ( ARF ) - guanine nucleotide exchange factors during the recycling of integrin beta1 .
	manualset3
98906	2	401011	13	NULL	NULL	0	NULL	roles	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigate the roles of the cytohesin ADP-ribosylation factor ( ARF ) - guanine nucleotide exchange factors during the recycling of integrin beta1 .
	manualset3
98907	3	401011	13	NULL	NULL	0	NULL	cytohesin ADP-ribosylation factor ( ARF ) - guanine nucleotide exchange factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigate the roles of the cytohesin ADP-ribosylation factor ( ARF ) - guanine nucleotide exchange factors during the recycling of integrin beta1 .
	manualset3
98908	4	401011	13	NULL	NULL	0	NULL	 recycling 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigate the roles of the cytohesin ADP-ribosylation factor ( ARF ) - guanine nucleotide exchange factors during the recycling of integrin beta1 .
	manualset3
98909	5	401011	13	NULL	NULL	0	NULL	integrin beta1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigate the roles of the cytohesin ADP-ribosylation factor ( ARF ) - guanine nucleotide exchange factors during the recycling of integrin beta1 .
	manualset3
98910	1	401012	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigated the effect of cathodal DC stimulation on spontaneous neural activity and on motor responses evoked by stimulation of the central and peripheral nervous system .
	manualset3
98911	2	401012	13	NULL	NULL	0	NULL	effect 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigated the effect of cathodal DC stimulation on spontaneous neural activity and on motor responses evoked by stimulation of the central and peripheral nervous system .
	manualset3
98912	3	401012	13	NULL	NULL	0	NULL	cathodal DC stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigated the effect of cathodal DC stimulation on spontaneous neural activity and on motor responses evoked by stimulation of the central and peripheral nervous system .
	manualset3
98913	4	401012	13	NULL	NULL	0	NULL	 neural activity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigated the effect of cathodal DC stimulation on spontaneous neural activity and on motor responses evoked by stimulation of the central and peripheral nervous system .
	manualset3
98914	5	401012	13	NULL	NULL	0	NULL	 motor responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigated the effect of cathodal DC stimulation on spontaneous neural activity and on motor responses evoked by stimulation of the central and peripheral nervous system .
	manualset3
98915	6	401012	13	NULL	NULL	0	NULL	stimulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigated the effect of cathodal DC stimulation on spontaneous neural activity and on motor responses evoked by stimulation of the central and peripheral nervous system .
	manualset3
98916	7	401012	13	NULL	NULL	0	NULL	 central nervous system	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigated the effect of cathodal DC stimulation on spontaneous neural activity and on motor responses evoked by stimulation of the central and peripheral nervous system .
	manualset3
98917	8	401012	13	NULL	NULL	0	NULL	peripheral nervous system	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigated the effect of cathodal DC stimulation on spontaneous neural activity and on motor responses evoked by stimulation of the central and peripheral nervous system .
	manualset3
98918	1	401013	13	NULL	NULL	0	NULL	2-fold increase	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2-fold increase of the number of cAMP binding sites .
	manualset3
98919	2	401013	13	NULL	NULL	0	NULL	 number	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2-fold increase of the number of cAMP binding sites .
	manualset3
98920	3	401013	13	NULL	NULL	0	NULL	cAMP binding sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	2-fold increase of the number of cAMP binding sites .
	manualset3
98921	1	401014	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigated the effects of preoperative oral carbohydrate administration on postoperative insulin resistance ( PIR ) , gastric fluid volume , preoperative discomfort , and variables of organ dysfunction in ASA physical status III-IV patients undergoing elective cardiac surgery , including those with noninsulin-dependent Type-2 diabetes mellitus .
	manualset3
98922	2	401014	13	NULL	NULL	0	NULL	effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigated the effects of preoperative oral carbohydrate administration on postoperative insulin resistance ( PIR ) , gastric fluid volume , preoperative discomfort , and variables of organ dysfunction in ASA physical status III-IV patients undergoing elective cardiac surgery , including those with noninsulin-dependent Type-2 diabetes mellitus .
	manualset3
98923	3	401014	13	NULL	NULL	0	NULL	preoperative oral carbohydrate administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigated the effects of preoperative oral carbohydrate administration on postoperative insulin resistance ( PIR ) , gastric fluid volume , preoperative discomfort , and variables of organ dysfunction in ASA physical status III-IV patients undergoing elective cardiac surgery , including those with noninsulin-dependent Type-2 diabetes mellitus .
	manualset3
98924	4	401014	13	NULL	NULL	0	NULL	postoperative insulin resistance ( PIR ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigated the effects of preoperative oral carbohydrate administration on postoperative insulin resistance ( PIR ) , gastric fluid volume , preoperative discomfort , and variables of organ dysfunction in ASA physical status III-IV patients undergoing elective cardiac surgery , including those with noninsulin-dependent Type-2 diabetes mellitus .
	manualset3
98925	5	401014	13	NULL	NULL	0	NULL	gastric fluid volume	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigated the effects of preoperative oral carbohydrate administration on postoperative insulin resistance ( PIR ) , gastric fluid volume , preoperative discomfort , and variables of organ dysfunction in ASA physical status III-IV patients undergoing elective cardiac surgery , including those with noninsulin-dependent Type-2 diabetes mellitus .
	manualset3
98926	6	401014	13	NULL	NULL	0	NULL	preoperative discomfort	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigated the effects of preoperative oral carbohydrate administration on postoperative insulin resistance ( PIR ) , gastric fluid volume , preoperative discomfort , and variables of organ dysfunction in ASA physical status III-IV patients undergoing elective cardiac surgery , including those with noninsulin-dependent Type-2 diabetes mellitus .
	manualset3
98927	7	401014	13	NULL	NULL	0	NULL	variables of organ dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigated the effects of preoperative oral carbohydrate administration on postoperative insulin resistance ( PIR ) , gastric fluid volume , preoperative discomfort , and variables of organ dysfunction in ASA physical status III-IV patients undergoing elective cardiac surgery , including those with noninsulin-dependent Type-2 diabetes mellitus .
	manualset3
98928	8	401014	13	NULL	NULL	0	NULL	ASA physical status III-IV patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigated the effects of preoperative oral carbohydrate administration on postoperative insulin resistance ( PIR ) , gastric fluid volume , preoperative discomfort , and variables of organ dysfunction in ASA physical status III-IV patients undergoing elective cardiac surgery , including those with noninsulin-dependent Type-2 diabetes mellitus .
	manualset3
98929	9	401014	13	NULL	NULL	0	NULL	 elective cardiac surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigated the effects of preoperative oral carbohydrate administration on postoperative insulin resistance ( PIR ) , gastric fluid volume , preoperative discomfort , and variables of organ dysfunction in ASA physical status III-IV patients undergoing elective cardiac surgery , including those with noninsulin-dependent Type-2 diabetes mellitus .
	manualset3
98930	10	401014	13	NULL	NULL	0	NULL	noninsulin-dependent Type-2 diabetes mellitus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigated the effects of preoperative oral carbohydrate administration on postoperative insulin resistance ( PIR ) , gastric fluid volume , preoperative discomfort , and variables of organ dysfunction in ASA physical status III-IV patients undergoing elective cardiac surgery , including those with noninsulin-dependent Type-2 diabetes mellitus .
	manualset3
98931	1	401015	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigated their role in human defense against the varicella zoster virus .
	manualset3
98932	2	401015	13	NULL	NULL	0	NULL	role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigated their role in human defense against the varicella zoster virus .
	manualset3
98933	3	401015	13	NULL	NULL	0	NULL	human defense	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigated their role in human defense against the varicella zoster virus .
	manualset3
98934	4	401015	13	NULL	NULL	0	NULL	varicella zoster virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigated their role in human defense against the varicella zoster virus .
	manualset3
98935	1	401016	13	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigated whether BzPO with or without Cu ( I ) caused promutagenic DNA damage in the supF gene of the mutation reporter plasmid pS189 replicating in human Ad293 cells .
	manualset3
98936	2	401016	13	NULL	NULL	0	NULL	 BzPO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigated whether BzPO with or without Cu ( I ) caused promutagenic DNA damage in the supF gene of the mutation reporter plasmid pS189 replicating in human Ad293 cells .
	manualset3
98937	3	401016	13	NULL	NULL	0	NULL	Cu ( I ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigated whether BzPO with or without Cu ( I ) caused promutagenic DNA damage in the supF gene of the mutation reporter plasmid pS189 replicating in human Ad293 cells .
	manualset3
98938	4	401016	13	NULL	NULL	0	NULL	promutagenic DNA damage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigated whether BzPO with or without Cu ( I ) caused promutagenic DNA damage in the supF gene of the mutation reporter plasmid pS189 replicating in human Ad293 cells .
	manualset3
98939	5	401016	13	NULL	NULL	0	NULL	supF gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigated whether BzPO with or without Cu ( I ) caused promutagenic DNA damage in the supF gene of the mutation reporter plasmid pS189 replicating in human Ad293 cells .
	manualset3
98940	6	401016	13	NULL	NULL	0	NULL	 mutation reporter plasmid pS189	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigated whether BzPO with or without Cu ( I ) caused promutagenic DNA damage in the supF gene of the mutation reporter plasmid pS189 replicating in human Ad293 cells .
	manualset3
98941	7	401016	13	NULL	NULL	0	NULL	replicating 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigated whether BzPO with or without Cu ( I ) caused promutagenic DNA damage in the supF gene of the mutation reporter plasmid pS189 replicating in human Ad293 cells .
	manualset3
98942	8	401016	13	NULL	NULL	0	NULL	human Ad293 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we investigated whether BzPO with or without Cu ( I ) caused promutagenic DNA damage in the supF gene of the mutation reporter plasmid pS189 replicating in human Ad293 cells .
	manualset3
98943	1	401017	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we showed that all HCC cell lines and clinical samples expressed high level of CD46 , the receptor for Adenovirus 35 ( Ad35 ) and constructed new fiber chimeric oncolytic adenoviruses with or without a p53 gene expression cassette , SG635-p53 and SG635 , respectively .
	manualset3
98944	2	401017	13	NULL	NULL	0	NULL	HCC cell lines 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we showed that all HCC cell lines and clinical samples expressed high level of CD46 , the receptor for Adenovirus 35 ( Ad35 ) and constructed new fiber chimeric oncolytic adenoviruses with or without a p53 gene expression cassette , SG635-p53 and SG635 , respectively .
	manualset3
98945	3	401017	13	NULL	NULL	0	NULL	 clinical samples 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we showed that all HCC cell lines and clinical samples expressed high level of CD46 , the receptor for Adenovirus 35 ( Ad35 ) and constructed new fiber chimeric oncolytic adenoviruses with or without a p53 gene expression cassette , SG635-p53 and SG635 , respectively .
	manualset3
98946	4	401017	13	NULL	NULL	0	NULL	high level	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we showed that all HCC cell lines and clinical samples expressed high level of CD46 , the receptor for Adenovirus 35 ( Ad35 ) and constructed new fiber chimeric oncolytic adenoviruses with or without a p53 gene expression cassette , SG635-p53 and SG635 , respectively .
	manualset3
98947	5	401017	13	NULL	NULL	0	NULL	 CD46	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we showed that all HCC cell lines and clinical samples expressed high level of CD46 , the receptor for Adenovirus 35 ( Ad35 ) and constructed new fiber chimeric oncolytic adenoviruses with or without a p53 gene expression cassette , SG635-p53 and SG635 , respectively .
	manualset3
98948	6	401017	13	NULL	NULL	0	NULL	receptor for Adenovirus 35 ( Ad35 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we showed that all HCC cell lines and clinical samples expressed high level of CD46 , the receptor for Adenovirus 35 ( Ad35 ) and constructed new fiber chimeric oncolytic adenoviruses with or without a p53 gene expression cassette , SG635-p53 and SG635 , respectively .
	manualset3
98949	7	401017	13	NULL	NULL	0	NULL	fiber chimeric oncolytic adenoviruses 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we showed that all HCC cell lines and clinical samples expressed high level of CD46 , the receptor for Adenovirus 35 ( Ad35 ) and constructed new fiber chimeric oncolytic adenoviruses with or without a p53 gene expression cassette , SG635-p53 and SG635 , respectively .
	manualset3
98950	8	401017	13	NULL	NULL	0	NULL	p53 gene expression cassette	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we showed that all HCC cell lines and clinical samples expressed high level of CD46 , the receptor for Adenovirus 35 ( Ad35 ) and constructed new fiber chimeric oncolytic adenoviruses with or without a p53 gene expression cassette , SG635-p53 and SG635 , respectively .
	manualset3
98951	9	401017	13	NULL	NULL	0	NULL	SG635-p53	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we showed that all HCC cell lines and clinical samples expressed high level of CD46 , the receptor for Adenovirus 35 ( Ad35 ) and constructed new fiber chimeric oncolytic adenoviruses with or without a p53 gene expression cassette , SG635-p53 and SG635 , respectively .
	manualset3
98952	10	401017	13	NULL	NULL	0	NULL	SG635 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we showed that all HCC cell lines and clinical samples expressed high level of CD46 , the receptor for Adenovirus 35 ( Ad35 ) and constructed new fiber chimeric oncolytic adenoviruses with or without a p53 gene expression cassette , SG635-p53 and SG635 , respectively .
	manualset3
98955	1	401018	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we showed that bacterial lipopolysaccharide ( LPS ) , which should activate B lymphocytes polyclonally , could not trigger an anti-H-2d plaque-forming cell response .
	manualset3
98956	2	401018	13	NULL	NULL	0	NULL	bacterial lipopolysaccharide ( LPS )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we showed that bacterial lipopolysaccharide ( LPS ) , which should activate B lymphocytes polyclonally , could not trigger an anti-H-2d plaque-forming cell response .
	manualset3
98958	3	401018	13	NULL	NULL	0	NULL	B lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we showed that bacterial lipopolysaccharide ( LPS ) , which should activate B lymphocytes polyclonally , could not trigger an anti-H-2d plaque-forming cell response .
	manualset3
98959	4	401018	13	NULL	NULL	0	NULL	anti-H-2d plaque-forming cell response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we showed that bacterial lipopolysaccharide ( LPS ) , which should activate B lymphocytes polyclonally , could not trigger an anti-H-2d plaque-forming cell response .
	manualset3
98960	1	401019	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we sought conditions to study the coccoid morphology of V. cholerae , and found that coccoid-shaped cells can express and produce the virulence factor toxin co-regulated pilus ( TCP ) and are able to colonize the infant mouse to the same extent as bacillus-shaped cells .
	manualset3
98961	2	401019	13	NULL	NULL	0	NULL	conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we sought conditions to study the coccoid morphology of V. cholerae , and found that coccoid-shaped cells can express and produce the virulence factor toxin co-regulated pilus ( TCP ) and are able to colonize the infant mouse to the same extent as bacillus-shaped cells .
	manualset3
98962	3	401019	13	NULL	NULL	0	NULL	coccoid morphology 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we sought conditions to study the coccoid morphology of V. cholerae , and found that coccoid-shaped cells can express and produce the virulence factor toxin co-regulated pilus ( TCP ) and are able to colonize the infant mouse to the same extent as bacillus-shaped cells .
	manualset3
98963	4	401019	13	NULL	NULL	0	NULL	V. cholerae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we sought conditions to study the coccoid morphology of V. cholerae , and found that coccoid-shaped cells can express and produce the virulence factor toxin co-regulated pilus ( TCP ) and are able to colonize the infant mouse to the same extent as bacillus-shaped cells .
	manualset3
98964	5	401019	13	NULL	NULL	0	NULL	coccoid-shaped cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we sought conditions to study the coccoid morphology of V. cholerae , and found that coccoid-shaped cells can express and produce the virulence factor toxin co-regulated pilus ( TCP ) and are able to colonize the infant mouse to the same extent as bacillus-shaped cells .
	manualset3
98965	6	401019	13	NULL	NULL	0	NULL	virulence factor toxin co-regulated pilus ( TCP ) 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we sought conditions to study the coccoid morphology of V. cholerae , and found that coccoid-shaped cells can express and produce the virulence factor toxin co-regulated pilus ( TCP ) and are able to colonize the infant mouse to the same extent as bacillus-shaped cells .
	manualset3
98966	7	401019	13	NULL	NULL	0	NULL	 infant mouse	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we sought conditions to study the coccoid morphology of V. cholerae , and found that coccoid-shaped cells can express and produce the virulence factor toxin co-regulated pilus ( TCP ) and are able to colonize the infant mouse to the same extent as bacillus-shaped cells .
	manualset3
98967	8	401019	13	NULL	NULL	0	NULL	same extent 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we sought conditions to study the coccoid morphology of V. cholerae , and found that coccoid-shaped cells can express and produce the virulence factor toxin co-regulated pilus ( TCP ) and are able to colonize the infant mouse to the same extent as bacillus-shaped cells .
	manualset3
98968	9	401019	13	NULL	NULL	0	NULL	bacillus-shaped cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we sought conditions to study the coccoid morphology of V. cholerae , and found that coccoid-shaped cells can express and produce the virulence factor toxin co-regulated pilus ( TCP ) and are able to colonize the infant mouse to the same extent as bacillus-shaped cells .
	manualset3
98969	1	401020	13	NULL	NULL	0	NULL	 study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we were unable to show any sensitization to epinephrine following xylazine administration during halothane anesthesia , while a protective effect was shown with a low dose of acepromazine .
	manualset3
98970	2	401020	13	NULL	NULL	0	NULL	sensitization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we were unable to show any sensitization to epinephrine following xylazine administration during halothane anesthesia , while a protective effect was shown with a low dose of acepromazine .
	manualset3
98971	3	401020	13	NULL	NULL	0	NULL	epinephrine 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we were unable to show any sensitization to epinephrine following xylazine administration during halothane anesthesia , while a protective effect was shown with a low dose of acepromazine .
	manualset3
98972	4	401020	13	NULL	NULL	0	NULL	xylazine administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we were unable to show any sensitization to epinephrine following xylazine administration during halothane anesthesia , while a protective effect was shown with a low dose of acepromazine .
	manualset3
98973	5	401020	13	NULL	NULL	0	NULL	halothane anesthesia	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we were unable to show any sensitization to epinephrine following xylazine administration during halothane anesthesia , while a protective effect was shown with a low dose of acepromazine .
	manualset3
98974	6	401020	13	NULL	NULL	0	NULL	protective effect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we were unable to show any sensitization to epinephrine following xylazine administration during halothane anesthesia , while a protective effect was shown with a low dose of acepromazine .
	manualset3
98975	7	401020	13	NULL	NULL	0	NULL	low dose of acepromazine	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study we were unable to show any sensitization to epinephrine following xylazine administration during halothane anesthesia , while a protective effect was shown with a low dose of acepromazine .
	manualset3
98976	1	401021	13	NULL	NULL	0	NULL	way 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this way , sustained lactation-associated metabolic changes are considered protective to women 's health .
	manualset3
98977	2	401021	13	NULL	NULL	0	NULL	lactation-associated metabolic changes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this way , sustained lactation-associated metabolic changes are considered protective to women 's health .
	manualset3
98978	3	401021	13	NULL	NULL	0	NULL	women 's health 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this way , sustained lactation-associated metabolic changes are considered protective to women 's health .
	manualset3
98979	1	401022	13	NULL	NULL	NULL	NULL	2.2 % of the total	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	2.2 % of the total polysomal RNA and the number average size was 1500 -- 1800 nucleotides , as judged by sedimentation analysis on sucrose density gradients containing Me2SO .
	manualset3
98980	2	401022	13	NULL	NULL	0	NULL	polysomal RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	2.2 % of the total polysomal RNA and the number average size was 1500 -- 1800 nucleotides , as judged by sedimentation analysis on sucrose density gradients containing Me2SO .
	manualset3
98981	3	401022	13	NULL	NULL	0	NULL	number average size	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2.2 % of the total polysomal RNA and the number average size was 1500 -- 1800 nucleotides , as judged by sedimentation analysis on sucrose density gradients containing Me2SO .
	manualset3
98982	4	401022	13	NULL	NULL	0	NULL	1500 -- 1800 nucleotides	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	2.2 % of the total polysomal RNA and the number average size was 1500 -- 1800 nucleotides , as judged by sedimentation analysis on sucrose density gradients containing Me2SO .
	manualset3
98983	5	401022	13	NULL	NULL	0	NULL	sedimentation analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	2.2 % of the total polysomal RNA and the number average size was 1500 -- 1800 nucleotides , as judged by sedimentation analysis on sucrose density gradients containing Me2SO .
	manualset3
98984	6	401022	13	NULL	NULL	0	NULL	sucrose density gradients 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2.2 % of the total polysomal RNA and the number average size was 1500 -- 1800 nucleotides , as judged by sedimentation analysis on sucrose density gradients containing Me2SO .
	manualset3
98985	7	401022	13	NULL	NULL	0	NULL	Me2SO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	2.2 % of the total polysomal RNA and the number average size was 1500 -- 1800 nucleotides , as judged by sedimentation analysis on sucrose density gradients containing Me2SO .
	manualset3
98986	1	401023	13	NULL	NULL	NULL	NULL	work	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this work , diverse hollow nanoparticles of metal oxides and sulfides were prepared by simply laser ablating metal targets in properly chosen liquids .
	manualset3
98987	2	401023	13	NULL	NULL	0	NULL	nanoparticles of metal oxides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , diverse hollow nanoparticles of metal oxides and sulfides were prepared by simply laser ablating metal targets in properly chosen liquids .
	manualset3
98988	3	401023	13	NULL	NULL	0	NULL	nanoparticles of sulfides	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , diverse hollow nanoparticles of metal oxides and sulfides were prepared by simply laser ablating metal targets in properly chosen liquids .
	manualset3
98989	4	401023	13	NULL	NULL	0	NULL	laser ablating metal targets	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , diverse hollow nanoparticles of metal oxides and sulfides were prepared by simply laser ablating metal targets in properly chosen liquids .
	manualset3
98990	5	401023	13	NULL	NULL	0	NULL	liquids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , diverse hollow nanoparticles of metal oxides and sulfides were prepared by simply laser ablating metal targets in properly chosen liquids .
	manualset3
98991	1	401024	13	NULL	NULL	0	NULL	work	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , eight different scoring functions have been combined with the aim of improving the prediction of protein-ligand binding conformations and affinities .
	manualset3
98992	2	401024	13	NULL	NULL	0	NULL	 eight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , eight different scoring functions have been combined with the aim of improving the prediction of protein-ligand binding conformations and affinities .
	manualset3
98993	3	401024	13	NULL	NULL	0	NULL	scoring functions	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , eight different scoring functions have been combined with the aim of improving the prediction of protein-ligand binding conformations and affinities .
	manualset3
98994	4	401024	13	NULL	NULL	0	NULL	aim	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , eight different scoring functions have been combined with the aim of improving the prediction of protein-ligand binding conformations and affinities .
	manualset3
98995	5	401024	13	NULL	NULL	0	NULL	prediction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , eight different scoring functions have been combined with the aim of improving the prediction of protein-ligand binding conformations and affinities .
	manualset3
98996	6	401024	13	NULL	NULL	0	NULL	protein-ligand binding conformations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , eight different scoring functions have been combined with the aim of improving the prediction of protein-ligand binding conformations and affinities .
	manualset3
98997	7	401024	13	NULL	NULL	0	NULL	protein-ligand binding affinities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , eight different scoring functions have been combined with the aim of improving the prediction of protein-ligand binding conformations and affinities .
	manualset3
98998	1	401025	13	NULL	NULL	0	NULL	work	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , molecular dynamics simulations are employed to provide further insight regarding the dependence of methane occupancy on the type of the LMGS and pressure .
	manualset3
98999	2	401025	13	NULL	NULL	0	NULL	molecular dynamics simulations 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , molecular dynamics simulations are employed to provide further insight regarding the dependence of methane occupancy on the type of the LMGS and pressure .
	manualset3
99000	3	401025	13	NULL	NULL	0	NULL	insight 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , molecular dynamics simulations are employed to provide further insight regarding the dependence of methane occupancy on the type of the LMGS and pressure .
	manualset3
99001	4	401025	13	NULL	NULL	0	NULL	dependence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , molecular dynamics simulations are employed to provide further insight regarding the dependence of methane occupancy on the type of the LMGS and pressure .
	manualset3
99002	5	401025	13	NULL	NULL	0	NULL	methane occupancy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , molecular dynamics simulations are employed to provide further insight regarding the dependence of methane occupancy on the type of the LMGS and pressure .
	manualset3
99003	6	401025	13	NULL	NULL	0	NULL	type of the LMGS	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , molecular dynamics simulations are employed to provide further insight regarding the dependence of methane occupancy on the type of the LMGS and pressure .
	manualset3
99004	7	401025	13	NULL	NULL	0	NULL	pressure	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , molecular dynamics simulations are employed to provide further insight regarding the dependence of methane occupancy on the type of the LMGS and pressure .
	manualset3
99005	1	401026	13	NULL	NULL	0	NULL	 work 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , the numerical model RT3D was modified and applied to evaluate the effect of aquifer characteristics and injection system design on contact and treatment efficiency .
	manualset3
99006	2	401026	13	NULL	NULL	0	NULL	numerical model RT3D	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , the numerical model RT3D was modified and applied to evaluate the effect of aquifer characteristics and injection system design on contact and treatment efficiency .
	manualset3
99007	3	401026	13	NULL	NULL	0	NULL	effect of aquifer characteristics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , the numerical model RT3D was modified and applied to evaluate the effect of aquifer characteristics and injection system design on contact and treatment efficiency .
	manualset3
99008	4	401026	13	NULL	NULL	0	NULL	injection system design 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , the numerical model RT3D was modified and applied to evaluate the effect of aquifer characteristics and injection system design on contact and treatment efficiency .
	manualset3
99009	5	401026	13	NULL	NULL	0	NULL	contact efficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , the numerical model RT3D was modified and applied to evaluate the effect of aquifer characteristics and injection system design on contact and treatment efficiency .
	manualset3
99010	6	401026	13	NULL	NULL	0	NULL	treatment efficiency 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , the numerical model RT3D was modified and applied to evaluate the effect of aquifer characteristics and injection system design on contact and treatment efficiency .
	manualset3
99011	1	401027	13	NULL	NULL	0	NULL	work 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we compare various protocols for preparation of Saccharomyces cerevisiae cells for immunoelectron microscopy , ranging from classical chemical fixation to high-pressure freezing followed by freeze-substitution in different kinds of substitution media .
	manualset3
99012	2	401027	13	NULL	NULL	0	NULL	protocols for preparation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we compare various protocols for preparation of Saccharomyces cerevisiae cells for immunoelectron microscopy , ranging from classical chemical fixation to high-pressure freezing followed by freeze-substitution in different kinds of substitution media .
	manualset3
99013	3	401027	13	NULL	NULL	0	NULL	Saccharomyces cerevisiae cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we compare various protocols for preparation of Saccharomyces cerevisiae cells for immunoelectron microscopy , ranging from classical chemical fixation to high-pressure freezing followed by freeze-substitution in different kinds of substitution media .
	manualset3
99014	4	401027	13	NULL	NULL	0	NULL	 immunoelectron microscopy 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we compare various protocols for preparation of Saccharomyces cerevisiae cells for immunoelectron microscopy , ranging from classical chemical fixation to high-pressure freezing followed by freeze-substitution in different kinds of substitution media .
	manualset3
99015	5	401027	13	NULL	NULL	0	NULL	classical chemical fixation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we compare various protocols for preparation of Saccharomyces cerevisiae cells for immunoelectron microscopy , ranging from classical chemical fixation to high-pressure freezing followed by freeze-substitution in different kinds of substitution media .
	manualset3
99016	6	401027	13	NULL	NULL	0	NULL	 high-pressure freezing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we compare various protocols for preparation of Saccharomyces cerevisiae cells for immunoelectron microscopy , ranging from classical chemical fixation to high-pressure freezing followed by freeze-substitution in different kinds of substitution media .
	manualset3
99017	7	401027	13	NULL	NULL	0	NULL	freeze-substitution	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we compare various protocols for preparation of Saccharomyces cerevisiae cells for immunoelectron microscopy , ranging from classical chemical fixation to high-pressure freezing followed by freeze-substitution in different kinds of substitution media .
	manualset3
99018	8	401027	13	NULL	NULL	0	NULL	 kinds of substitution media	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we compare various protocols for preparation of Saccharomyces cerevisiae cells for immunoelectron microscopy , ranging from classical chemical fixation to high-pressure freezing followed by freeze-substitution in different kinds of substitution media .
	manualset3
99019	1	401028	13	NULL	NULL	0	NULL	work	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we conjugated recombinant adeno-associated virus serotype 2 ( rAAV2 ) to a heparinized small intestinal submucosa ( H-SIS ) matrix , which resulted in vector transduction upon cellular adhesion .
	manualset3
99020	2	401028	13	NULL	NULL	0	NULL	recombinant adeno-associated virus serotype 2 ( rAAV2 ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we conjugated recombinant adeno-associated virus serotype 2 ( rAAV2 ) to a heparinized small intestinal submucosa ( H-SIS ) matrix , which resulted in vector transduction upon cellular adhesion .
	manualset3
99021	3	401028	13	NULL	NULL	0	NULL	small intestinal submucosa ( H-SIS ) matrix	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we conjugated recombinant adeno-associated virus serotype 2 ( rAAV2 ) to a heparinized small intestinal submucosa ( H-SIS ) matrix , which resulted in vector transduction upon cellular adhesion .
	manualset3
99022	4	401028	13	NULL	NULL	0	NULL	vector transduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we conjugated recombinant adeno-associated virus serotype 2 ( rAAV2 ) to a heparinized small intestinal submucosa ( H-SIS ) matrix , which resulted in vector transduction upon cellular adhesion .
	manualset3
99023	5	401028	13	NULL	NULL	0	NULL	cellular adhesion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we conjugated recombinant adeno-associated virus serotype 2 ( rAAV2 ) to a heparinized small intestinal submucosa ( H-SIS ) matrix , which resulted in vector transduction upon cellular adhesion .
	manualset3
99024	1	401029	13	NULL	NULL	0	NULL	 work	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we describe the use of an actuated manipulator to physically manipulate such sensors to scan an area of interest generating 1-D scans while registering them to a guiding modality .
	manualset3
99025	2	401029	13	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we describe the use of an actuated manipulator to physically manipulate such sensors to scan an area of interest generating 1-D scans while registering them to a guiding modality .
	manualset3
99026	3	401029	13	NULL	NULL	0	NULL	manipulator	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we describe the use of an actuated manipulator to physically manipulate such sensors to scan an area of interest generating 1-D scans while registering them to a guiding modality .
	manualset3
99027	4	401029	13	NULL	NULL	0	NULL	sensors	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we describe the use of an actuated manipulator to physically manipulate such sensors to scan an area of interest generating 1-D scans while registering them to a guiding modality .
	manualset3
99028	5	401029	13	NULL	NULL	0	NULL	area	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we describe the use of an actuated manipulator to physically manipulate such sensors to scan an area of interest generating 1-D scans while registering them to a guiding modality .
	manualset3
99029	6	401029	13	NULL	NULL	0	NULL	interest	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we describe the use of an actuated manipulator to physically manipulate such sensors to scan an area of interest generating 1-D scans while registering them to a guiding modality .
	manualset3
99030	7	401029	13	NULL	NULL	0	NULL	1-D scans	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we describe the use of an actuated manipulator to physically manipulate such sensors to scan an area of interest generating 1-D scans while registering them to a guiding modality .
	manualset3
99031	8	401029	13	NULL	NULL	0	NULL	modality 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we describe the use of an actuated manipulator to physically manipulate such sensors to scan an area of interest generating 1-D scans while registering them to a guiding modality .
	manualset3
99032	1	401030	13	NULL	NULL	0	NULL	work	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we embed the classic kinship theory within an island model of population structure and allow for diverse demographic and life-history features to affect the direction of selection on imprinting .
	manualset3
99033	2	401030	13	NULL	NULL	0	NULL	classic kinship theory	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we embed the classic kinship theory within an island model of population structure and allow for diverse demographic and life-history features to affect the direction of selection on imprinting .
	manualset3
99034	3	401030	13	NULL	NULL	0	NULL	island model of population structure	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we embed the classic kinship theory within an island model of population structure and allow for diverse demographic and life-history features to affect the direction of selection on imprinting .
	manualset3
99035	4	401030	13	NULL	NULL	NULL	NULL	demographic features 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this work , we embed the classic kinship theory within an island model of population structure and allow for diverse demographic and life-history features to affect the direction of selection on imprinting .
	manualset3
99036	5	401030	13	NULL	NULL	0	NULL	life-history features 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we embed the classic kinship theory within an island model of population structure and allow for diverse demographic and life-history features to affect the direction of selection on imprinting .
	manualset3
99037	6	401030	13	NULL	NULL	0	NULL	direction of selection on imprinting	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we embed the classic kinship theory within an island model of population structure and allow for diverse demographic and life-history features to affect the direction of selection on imprinting .
	manualset3
99038	1	401031	13	NULL	NULL	0	NULL	work	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we propose to extend our optimization principle into a more general one , which includes the notion of information as defined by Shannon .
	manualset3
99039	2	401031	13	NULL	NULL	0	NULL	optimization principle	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we propose to extend our optimization principle into a more general one , which includes the notion of information as defined by Shannon .
	manualset3
99040	3	401031	13	NULL	NULL	0	NULL	notion of information 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we propose to extend our optimization principle into a more general one , which includes the notion of information as defined by Shannon .
	manualset3
99041	4	401031	13	NULL	NULL	0	NULL	Shannon	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we propose to extend our optimization principle into a more general one , which includes the notion of information as defined by Shannon .
	manualset3
99042	1	401032	13	NULL	NULL	0	NULL	 work 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we trace the instability to the nonanalytic character of the underlying spectrum and show that a correct splitting of the Hamiltonian , which renders the spectrum analytic , restores stability .
	manualset3
99044	3	401032	13	NULL	NULL	0	NULL	instability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we trace the instability to the nonanalytic character of the underlying spectrum and show that a correct splitting of the Hamiltonian , which renders the spectrum analytic , restores stability .
	manualset3
99045	4	401032	13	NULL	NULL	0	NULL	 nonanalytic character	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we trace the instability to the nonanalytic character of the underlying spectrum and show that a correct splitting of the Hamiltonian , which renders the spectrum analytic , restores stability .
	manualset3
99046	5	401032	13	NULL	NULL	0	NULL	spectrum	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we trace the instability to the nonanalytic character of the underlying spectrum and show that a correct splitting of the Hamiltonian , which renders the spectrum analytic , restores stability .
	manualset3
99047	6	401032	13	NULL	NULL	0	NULL	 splitting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we trace the instability to the nonanalytic character of the underlying spectrum and show that a correct splitting of the Hamiltonian , which renders the spectrum analytic , restores stability .
	manualset3
99048	7	401032	13	NULL	NULL	0	NULL	Hamiltonian	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we trace the instability to the nonanalytic character of the underlying spectrum and show that a correct splitting of the Hamiltonian , which renders the spectrum analytic , restores stability .
	manualset3
99049	8	401032	13	NULL	NULL	0	NULL	spectrum	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we trace the instability to the nonanalytic character of the underlying spectrum and show that a correct splitting of the Hamiltonian , which renders the spectrum analytic , restores stability .
	manualset3
99050	9	401032	13	NULL	NULL	0	NULL	stability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work , we trace the instability to the nonanalytic character of the underlying spectrum and show that a correct splitting of the Hamiltonian , which renders the spectrum analytic , restores stability .
	manualset3
99051	1	401033	13	NULL	NULL	0	NULL	work	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work 281 strains of bifidobacteria were anaerobically isolated from human faecal samples , supplied by volunteers of different ages ( youngs , adults , elders ) , and preliminarly described by microscopic observation .
	manualset3
99052	2	401033	13	NULL	NULL	0	NULL	281 strains	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work 281 strains of bifidobacteria were anaerobically isolated from human faecal samples , supplied by volunteers of different ages ( youngs , adults , elders ) , and preliminarly described by microscopic observation .
	manualset3
99053	3	401033	13	NULL	NULL	0	NULL	bifidobacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work 281 strains of bifidobacteria were anaerobically isolated from human faecal samples , supplied by volunteers of different ages ( youngs , adults , elders ) , and preliminarly described by microscopic observation .
	manualset3
99054	4	401033	13	NULL	NULL	0	NULL	human faecal samples	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work 281 strains of bifidobacteria were anaerobically isolated from human faecal samples , supplied by volunteers of different ages ( youngs , adults , elders ) , and preliminarly described by microscopic observation .
	manualset3
99055	5	401033	13	NULL	NULL	0	NULL	volunteers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work 281 strains of bifidobacteria were anaerobically isolated from human faecal samples , supplied by volunteers of different ages ( youngs , adults , elders ) , and preliminarly described by microscopic observation .
	manualset3
99056	6	401033	13	NULL	NULL	0	NULL	different ages	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work 281 strains of bifidobacteria were anaerobically isolated from human faecal samples , supplied by volunteers of different ages ( youngs , adults , elders ) , and preliminarly described by microscopic observation .
	manualset3
99057	7	401033	13	NULL	NULL	0	NULL	youngs	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work 281 strains of bifidobacteria were anaerobically isolated from human faecal samples , supplied by volunteers of different ages ( youngs , adults , elders ) , and preliminarly described by microscopic observation .
	manualset3
99058	8	401033	13	NULL	NULL	0	NULL	adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work 281 strains of bifidobacteria were anaerobically isolated from human faecal samples , supplied by volunteers of different ages ( youngs , adults , elders ) , and preliminarly described by microscopic observation .
	manualset3
99059	9	401033	13	NULL	NULL	0	NULL	elders	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work 281 strains of bifidobacteria were anaerobically isolated from human faecal samples , supplied by volunteers of different ages ( youngs , adults , elders ) , and preliminarly described by microscopic observation .
	manualset3
99060	10	401033	13	NULL	NULL	0	NULL	microscopic observation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work 281 strains of bifidobacteria were anaerobically isolated from human faecal samples , supplied by volunteers of different ages ( youngs , adults , elders ) , and preliminarly described by microscopic observation .
	manualset3
99061	1	401034	13	NULL	NULL	0	NULL	work 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work solid-state techniques , diffuse reflectance infrared Fourier transform spectroscopy ( DRIFTS ) and X-ray powder diffractometry ( XRPD ) were combined to analyze polymorphic purity of crystalline ranitidine-HCl , an antiulcer drug , H2 receptor antagonists .
	manualset3
99062	2	401034	13	NULL	NULL	0	NULL	 solid-state techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work solid-state techniques , diffuse reflectance infrared Fourier transform spectroscopy ( DRIFTS ) and X-ray powder diffractometry ( XRPD ) were combined to analyze polymorphic purity of crystalline ranitidine-HCl , an antiulcer drug , H2 receptor antagonists .
	manualset3
99063	3	401034	13	NULL	NULL	0	NULL	diffuse reflectance infrared Fourier transform spectroscopy ( DRIFTS )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work solid-state techniques , diffuse reflectance infrared Fourier transform spectroscopy ( DRIFTS ) and X-ray powder diffractometry ( XRPD ) were combined to analyze polymorphic purity of crystalline ranitidine-HCl , an antiulcer drug , H2 receptor antagonists .
	manualset3
99064	4	401034	13	NULL	NULL	0	NULL	X-ray powder diffractometry ( XRPD ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work solid-state techniques , diffuse reflectance infrared Fourier transform spectroscopy ( DRIFTS ) and X-ray powder diffractometry ( XRPD ) were combined to analyze polymorphic purity of crystalline ranitidine-HCl , an antiulcer drug , H2 receptor antagonists .
	manualset3
99065	5	401034	13	NULL	NULL	0	NULL	polymorphic purity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work solid-state techniques , diffuse reflectance infrared Fourier transform spectroscopy ( DRIFTS ) and X-ray powder diffractometry ( XRPD ) were combined to analyze polymorphic purity of crystalline ranitidine-HCl , an antiulcer drug , H2 receptor antagonists .
	manualset3
99066	6	401034	13	NULL	NULL	0	NULL	crystalline ranitidine-HCl 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work solid-state techniques , diffuse reflectance infrared Fourier transform spectroscopy ( DRIFTS ) and X-ray powder diffractometry ( XRPD ) were combined to analyze polymorphic purity of crystalline ranitidine-HCl , an antiulcer drug , H2 receptor antagonists .
	manualset3
99067	7	401034	13	NULL	NULL	0	NULL	antiulcer drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work solid-state techniques , diffuse reflectance infrared Fourier transform spectroscopy ( DRIFTS ) and X-ray powder diffractometry ( XRPD ) were combined to analyze polymorphic purity of crystalline ranitidine-HCl , an antiulcer drug , H2 receptor antagonists .
	manualset3
99068	8	401034	13	NULL	NULL	0	NULL	H2 receptor antagonists	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work solid-state techniques , diffuse reflectance infrared Fourier transform spectroscopy ( DRIFTS ) and X-ray powder diffractometry ( XRPD ) were combined to analyze polymorphic purity of crystalline ranitidine-HCl , an antiulcer drug , H2 receptor antagonists .
	manualset3
99143	1	401035	13	NULL	NULL	0	NULL	 work 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work this molecule was more extensively studied and diazoxide was used as reference mito-K ( ATP ) opener .
	manualset3
99144	2	401035	13	NULL	NULL	0	NULL	molecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work this molecule was more extensively studied and diazoxide was used as reference mito-K ( ATP ) opener .
	manualset3
99145	3	401035	13	NULL	NULL	0	NULL	diazoxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work this molecule was more extensively studied and diazoxide was used as reference mito-K ( ATP ) opener .
	manualset3
99146	4	401035	13	NULL	NULL	0	NULL	reference mito-K ( ATP ) opener	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work this molecule was more extensively studied and diazoxide was used as reference mito-K ( ATP ) opener .
	manualset3
99147	1	401036	13	NULL	NULL	0	NULL	work	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work we aimed to test the effects of testosterone on sex ratio of bovine embryos produced in vitro and to determine whether effects of sex and temperature are effectively decoupled in mammals .
	manualset3
99148	2	401036	13	NULL	NULL	0	NULL	effects of testosterone	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work we aimed to test the effects of testosterone on sex ratio of bovine embryos produced in vitro and to determine whether effects of sex and temperature are effectively decoupled in mammals .
	manualset3
99150	3	401036	13	NULL	NULL	0	NULL	sex ratio 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work we aimed to test the effects of testosterone on sex ratio of bovine embryos produced in vitro and to determine whether effects of sex and temperature are effectively decoupled in mammals .
	manualset3
99151	4	401036	13	NULL	NULL	0	NULL	 bovine embryos	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work we aimed to test the effects of testosterone on sex ratio of bovine embryos produced in vitro and to determine whether effects of sex and temperature are effectively decoupled in mammals .
	manualset3
99152	5	401036	13	NULL	NULL	0	NULL	effects of sex 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work we aimed to test the effects of testosterone on sex ratio of bovine embryos produced in vitro and to determine whether effects of sex and temperature are effectively decoupled in mammals .
	manualset3
99153	6	401036	13	NULL	NULL	0	NULL	effects of temperature	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work we aimed to test the effects of testosterone on sex ratio of bovine embryos produced in vitro and to determine whether effects of sex and temperature are effectively decoupled in mammals .
	manualset3
99154	7	401036	13	NULL	NULL	0	NULL	mammals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work we aimed to test the effects of testosterone on sex ratio of bovine embryos produced in vitro and to determine whether effects of sex and temperature are effectively decoupled in mammals .
	manualset3
99155	1	401037	13	NULL	NULL	0	NULL	work 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work we passivated small carbon nanoparticles by a combination of the surface-doping with nanoscale semiconductors and the organic functionalization , coupled with gel column fractionation to harvest the most fluorescent carbon dots , which exhibited fluorescence emission quantum yields of up to 78 % .
	manualset3
99156	2	401037	13	NULL	NULL	0	NULL	carbon nanoparticles	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work we passivated small carbon nanoparticles by a combination of the surface-doping with nanoscale semiconductors and the organic functionalization , coupled with gel column fractionation to harvest the most fluorescent carbon dots , which exhibited fluorescence emission quantum yields of up to 78 % .
	manualset3
99157	3	401037	13	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work we passivated small carbon nanoparticles by a combination of the surface-doping with nanoscale semiconductors and the organic functionalization , coupled with gel column fractionation to harvest the most fluorescent carbon dots , which exhibited fluorescence emission quantum yields of up to 78 % .
	manualset3
99158	4	401037	13	NULL	NULL	0	NULL	surface-doping	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work we passivated small carbon nanoparticles by a combination of the surface-doping with nanoscale semiconductors and the organic functionalization , coupled with gel column fractionation to harvest the most fluorescent carbon dots , which exhibited fluorescence emission quantum yields of up to 78 % .
	manualset3
99159	5	401037	13	NULL	NULL	0	NULL	nanoscale semiconductors	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work we passivated small carbon nanoparticles by a combination of the surface-doping with nanoscale semiconductors and the organic functionalization , coupled with gel column fractionation to harvest the most fluorescent carbon dots , which exhibited fluorescence emission quantum yields of up to 78 % .
	manualset3
99160	6	401037	13	NULL	NULL	0	NULL	organic functionalization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work we passivated small carbon nanoparticles by a combination of the surface-doping with nanoscale semiconductors and the organic functionalization , coupled with gel column fractionation to harvest the most fluorescent carbon dots , which exhibited fluorescence emission quantum yields of up to 78 % .
	manualset3
99161	7	401037	13	NULL	NULL	0	NULL	gel column fractionation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work we passivated small carbon nanoparticles by a combination of the surface-doping with nanoscale semiconductors and the organic functionalization , coupled with gel column fractionation to harvest the most fluorescent carbon dots , which exhibited fluorescence emission quantum yields of up to 78 % .
	manualset3
99162	8	401037	13	NULL	NULL	0	NULL	fluorescent carbon dots	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work we passivated small carbon nanoparticles by a combination of the surface-doping with nanoscale semiconductors and the organic functionalization , coupled with gel column fractionation to harvest the most fluorescent carbon dots , which exhibited fluorescence emission quantum yields of up to 78 % .
	manualset3
99163	9	401037	13	NULL	NULL	0	NULL	fluorescence emission quantum	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work we passivated small carbon nanoparticles by a combination of the surface-doping with nanoscale semiconductors and the organic functionalization , coupled with gel column fractionation to harvest the most fluorescent carbon dots , which exhibited fluorescence emission quantum yields of up to 78 % .
	manualset3
99164	10	401037	13	NULL	NULL	0	NULL	78 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work we passivated small carbon nanoparticles by a combination of the surface-doping with nanoscale semiconductors and the organic functionalization , coupled with gel column fractionation to harvest the most fluorescent carbon dots , which exhibited fluorescence emission quantum yields of up to 78 % .
	manualset3
99165	1	401038	13	NULL	NULL	0	NULL	work	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work we sequenced the whole genome of different passages of the YFV-17D strain used by Crucell Switzerland AG for vaccine production .
	manualset3
99166	2	401038	13	NULL	NULL	0	NULL	genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work we sequenced the whole genome of different passages of the YFV-17D strain used by Crucell Switzerland AG for vaccine production .
	manualset3
99167	3	401038	13	NULL	NULL	0	NULL	passages	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work we sequenced the whole genome of different passages of the YFV-17D strain used by Crucell Switzerland AG for vaccine production .
	manualset3
99168	4	401038	13	NULL	NULL	0	NULL	 YFV-17D strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work we sequenced the whole genome of different passages of the YFV-17D strain used by Crucell Switzerland AG for vaccine production .
	manualset3
99169	5	401038	13	NULL	NULL	0	NULL	Crucell Switzerland AG	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work we sequenced the whole genome of different passages of the YFV-17D strain used by Crucell Switzerland AG for vaccine production .
	manualset3
99170	6	401038	13	NULL	NULL	0	NULL	vaccine production	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In this work we sequenced the whole genome of different passages of the YFV-17D strain used by Crucell Switzerland AG for vaccine production .
	manualset3
99171	1	401039	13	NULL	NULL	0	NULL	2 ' , 3 ' - O - ( 2 , 4 , 6-trinitrophenyl ) -8 - azido-AMP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ' , 3 ' - O - ( 2 , 4 , 6-trinitrophenyl ) -8 - azido-AMP ( TNP-8N3-AMP ) and - ATP photolabel Lys-492 at the active site of the Ca ( 2 + ) - ATPase of sarcoplasmic reticulum ( McIntosh , D. B. , Woolley , D. G. , and Berman , M. C. ( 1992 ) J. Biol .
	manualset3
99172	2	401039	13	NULL	NULL	0	NULL	TNP-8N3-AMP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ' , 3 ' - O - ( 2 , 4 , 6-trinitrophenyl ) -8 - azido-AMP ( TNP-8N3-AMP ) and - ATP photolabel Lys-492 at the active site of the Ca ( 2 + ) - ATPase of sarcoplasmic reticulum ( McIntosh , D. B. , Woolley , D. G. , and Berman , M. C. ( 1992 ) J. Biol .
	manualset3
99173	3	401039	13	NULL	NULL	0	NULL	2 ' , 3 ' - O - ( 2 , 4 , 6-trinitrophenyl ) -8 - azido-ATP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ' , 3 ' - O - ( 2 , 4 , 6-trinitrophenyl ) -8 - azido-AMP ( TNP-8N3-AMP ) and - ATP photolabel Lys-492 at the active site of the Ca ( 2 + ) - ATPase of sarcoplasmic reticulum ( McIntosh , D. B. , Woolley , D. G. , and Berman , M. C. ( 1992 ) J. Biol .
	manualset3
99174	4	401039	13	NULL	NULL	NULL	NULL	photolabel 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	2 ' , 3 ' - O - ( 2 , 4 , 6-trinitrophenyl ) -8 - azido-AMP ( TNP-8N3-AMP ) and - ATP photolabel Lys-492 at the active site of the Ca ( 2 + ) - ATPase of sarcoplasmic reticulum ( McIntosh , D. B. , Woolley , D. G. , and Berman , M. C. ( 1992 ) J. Biol .
	manualset3
99175	5	401039	13	NULL	NULL	0	NULL	Lys-492	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ' , 3 ' - O - ( 2 , 4 , 6-trinitrophenyl ) -8 - azido-AMP ( TNP-8N3-AMP ) and - ATP photolabel Lys-492 at the active site of the Ca ( 2 + ) - ATPase of sarcoplasmic reticulum ( McIntosh , D. B. , Woolley , D. G. , and Berman , M. C. ( 1992 ) J. Biol .
	manualset3
99176	6	401039	13	NULL	NULL	0	NULL	active site of the Ca ( 2 + ) - ATPase 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ' , 3 ' - O - ( 2 , 4 , 6-trinitrophenyl ) -8 - azido-AMP ( TNP-8N3-AMP ) and - ATP photolabel Lys-492 at the active site of the Ca ( 2 + ) - ATPase of sarcoplasmic reticulum ( McIntosh , D. B. , Woolley , D. G. , and Berman , M. C. ( 1992 ) J. Biol .
	manualset3
99177	7	401039	13	NULL	NULL	0	NULL	sarcoplasmic reticulum	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ' , 3 ' - O - ( 2 , 4 , 6-trinitrophenyl ) -8 - azido-AMP ( TNP-8N3-AMP ) and - ATP photolabel Lys-492 at the active site of the Ca ( 2 + ) - ATPase of sarcoplasmic reticulum ( McIntosh , D. B. , Woolley , D. G. , and Berman , M. C. ( 1992 ) J. Biol .
	manualset3
99178	8	401039	13	NULL	NULL	0	NULL	McIntosh , D. B.	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ' , 3 ' - O - ( 2 , 4 , 6-trinitrophenyl ) -8 - azido-AMP ( TNP-8N3-AMP ) and - ATP photolabel Lys-492 at the active site of the Ca ( 2 + ) - ATPase of sarcoplasmic reticulum ( McIntosh , D. B. , Woolley , D. G. , and Berman , M. C. ( 1992 ) J. Biol .
	manualset3
99179	9	401039	13	NULL	NULL	0	NULL	Woolley , D. G.	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ' , 3 ' - O - ( 2 , 4 , 6-trinitrophenyl ) -8 - azido-AMP ( TNP-8N3-AMP ) and - ATP photolabel Lys-492 at the active site of the Ca ( 2 + ) - ATPase of sarcoplasmic reticulum ( McIntosh , D. B. , Woolley , D. G. , and Berman , M. C. ( 1992 ) J. Biol .
	manualset3
99180	10	401039	13	NULL	NULL	0	NULL	Berman , M. C. 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ' , 3 ' - O - ( 2 , 4 , 6-trinitrophenyl ) -8 - azido-AMP ( TNP-8N3-AMP ) and - ATP photolabel Lys-492 at the active site of the Ca ( 2 + ) - ATPase of sarcoplasmic reticulum ( McIntosh , D. B. , Woolley , D. G. , and Berman , M. C. ( 1992 ) J. Biol .
	manualset3
99181	11	401039	13	NULL	NULL	0	NULL	1992	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ' , 3 ' - O - ( 2 , 4 , 6-trinitrophenyl ) -8 - azido-AMP ( TNP-8N3-AMP ) and - ATP photolabel Lys-492 at the active site of the Ca ( 2 + ) - ATPase of sarcoplasmic reticulum ( McIntosh , D. B. , Woolley , D. G. , and Berman , M. C. ( 1992 ) J. Biol .
	manualset3
99182	12	401039	13	NULL	NULL	0	NULL	J. Biol 	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ' , 3 ' - O - ( 2 , 4 , 6-trinitrophenyl ) -8 - azido-AMP ( TNP-8N3-AMP ) and - ATP photolabel Lys-492 at the active site of the Ca ( 2 + ) - ATPase of sarcoplasmic reticulum ( McIntosh , D. B. , Woolley , D. G. , and Berman , M. C. ( 1992 ) J. Biol .
	manualset3
99183	1	401040	13	NULL	NULL	0	NULL	 TPN	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	In those receiving TPN and metronidazole , serum activities of alkaline phosphatase and gamma-glutamyl-transferase decreased or remained normal after 30 days of TPN .
	manualset3
99184	2	401040	13	NULL	NULL	0	NULL	metronidazole 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In those receiving TPN and metronidazole , serum activities of alkaline phosphatase and gamma-glutamyl-transferase decreased or remained normal after 30 days of TPN .
	manualset3
99185	3	401040	13	NULL	NULL	0	NULL	serum activities 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In those receiving TPN and metronidazole , serum activities of alkaline phosphatase and gamma-glutamyl-transferase decreased or remained normal after 30 days of TPN .
	manualset3
99186	4	401040	13	NULL	NULL	0	NULL	alkaline phosphatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In those receiving TPN and metronidazole , serum activities of alkaline phosphatase and gamma-glutamyl-transferase decreased or remained normal after 30 days of TPN .
	manualset3
99187	5	401040	13	NULL	NULL	0	NULL	 gamma-glutamyl-transferase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In those receiving TPN and metronidazole , serum activities of alkaline phosphatase and gamma-glutamyl-transferase decreased or remained normal after 30 days of TPN .
	manualset3
99188	6	401040	13	NULL	NULL	0	NULL	 30 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In those receiving TPN and metronidazole , serum activities of alkaline phosphatase and gamma-glutamyl-transferase decreased or remained normal after 30 days of TPN .
	manualset3
99189	7	401040	13	NULL	NULL	0	NULL	TPN	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	In those receiving TPN and metronidazole , serum activities of alkaline phosphatase and gamma-glutamyl-transferase decreased or remained normal after 30 days of TPN .
	manualset3
99190	1	401041	13	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In three patients , O2 desaturation was easily managed by transient reversion of the effects of meperidine or fentanyl with naloxone .
	manualset3
99191	2	401041	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In three patients , O2 desaturation was easily managed by transient reversion of the effects of meperidine or fentanyl with naloxone .
	manualset3
99192	3	401041	13	NULL	NULL	0	NULL	O2 desaturation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In three patients , O2 desaturation was easily managed by transient reversion of the effects of meperidine or fentanyl with naloxone .
	manualset3
99193	4	401041	13	NULL	NULL	0	NULL	transient reversion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In three patients , O2 desaturation was easily managed by transient reversion of the effects of meperidine or fentanyl with naloxone .
	manualset3
99194	5	401041	13	NULL	NULL	0	NULL	 effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In three patients , O2 desaturation was easily managed by transient reversion of the effects of meperidine or fentanyl with naloxone .
	manualset3
99195	6	401041	13	NULL	NULL	0	NULL	 meperidine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In three patients , O2 desaturation was easily managed by transient reversion of the effects of meperidine or fentanyl with naloxone .
	manualset3
99196	7	401041	13	NULL	NULL	0	NULL	 fentanyl	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In three patients , O2 desaturation was easily managed by transient reversion of the effects of meperidine or fentanyl with naloxone .
	manualset3
99197	8	401041	13	NULL	NULL	0	NULL	naloxone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In three patients , O2 desaturation was easily managed by transient reversion of the effects of meperidine or fentanyl with naloxone .
	manualset3
99198	1	401042	13	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In three studies , we focus particularly on essentialist entitativity ( EE , referring to beliefs about the uniformity , informativeness , and inherent core of racial groups ) , probing into its relationships with epistemic need for closure ( NFC ) and prejudice .
	manualset3
99199	2	401042	13	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In three studies , we focus particularly on essentialist entitativity ( EE , referring to beliefs about the uniformity , informativeness , and inherent core of racial groups ) , probing into its relationships with epistemic need for closure ( NFC ) and prejudice .
	manualset3
99200	3	401042	13	NULL	NULL	0	NULL	essentialist entitativity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In three studies , we focus particularly on essentialist entitativity ( EE , referring to beliefs about the uniformity , informativeness , and inherent core of racial groups ) , probing into its relationships with epistemic need for closure ( NFC ) and prejudice .
	manualset3
99201	4	401042	13	NULL	NULL	0	NULL	 EE	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In three studies , we focus particularly on essentialist entitativity ( EE , referring to beliefs about the uniformity , informativeness , and inherent core of racial groups ) , probing into its relationships with epistemic need for closure ( NFC ) and prejudice .
	manualset3
99202	5	401042	13	NULL	NULL	0	NULL	beliefs 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In three studies , we focus particularly on essentialist entitativity ( EE , referring to beliefs about the uniformity , informativeness , and inherent core of racial groups ) , probing into its relationships with epistemic need for closure ( NFC ) and prejudice .
	manualset3
99203	6	401042	13	NULL	NULL	0	NULL	uniformity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In three studies , we focus particularly on essentialist entitativity ( EE , referring to beliefs about the uniformity , informativeness , and inherent core of racial groups ) , probing into its relationships with epistemic need for closure ( NFC ) and prejudice .
	manualset3
99204	7	401042	13	NULL	NULL	0	NULL	informativeness 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In three studies , we focus particularly on essentialist entitativity ( EE , referring to beliefs about the uniformity , informativeness , and inherent core of racial groups ) , probing into its relationships with epistemic need for closure ( NFC ) and prejudice .
	manualset3
99205	8	401042	13	NULL	NULL	0	NULL	inherent core 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In three studies , we focus particularly on essentialist entitativity ( EE , referring to beliefs about the uniformity , informativeness , and inherent core of racial groups ) , probing into its relationships with epistemic need for closure ( NFC ) and prejudice .
	manualset3
99206	9	401042	13	NULL	NULL	0	NULL	 racial groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In three studies , we focus particularly on essentialist entitativity ( EE , referring to beliefs about the uniformity , informativeness , and inherent core of racial groups ) , probing into its relationships with epistemic need for closure ( NFC ) and prejudice .
	manualset3
99207	10	401042	13	NULL	NULL	0	NULL	relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In three studies , we focus particularly on essentialist entitativity ( EE , referring to beliefs about the uniformity , informativeness , and inherent core of racial groups ) , probing into its relationships with epistemic need for closure ( NFC ) and prejudice .
	manualset3
99208	11	401042	13	NULL	NULL	0	NULL	epistemic need for closure ( NFC )	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In three studies , we focus particularly on essentialist entitativity ( EE , referring to beliefs about the uniformity , informativeness , and inherent core of racial groups ) , probing into its relationships with epistemic need for closure ( NFC ) and prejudice .
	manualset3
99209	12	401042	13	NULL	NULL	0	NULL	prejudice	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In three studies , we focus particularly on essentialist entitativity ( EE , referring to beliefs about the uniformity , informativeness , and inherent core of racial groups ) , probing into its relationships with epistemic need for closure ( NFC ) and prejudice .
	manualset3
99210	1	401043	13	NULL	NULL	0	NULL	 transferase activity assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In transferase activity assay , a donor with high expression of B had increased B transferase activity in her serum , which suggested that the high-expression phenotype might be under the control of the glycosyltransferase gene .
	manualset3
99211	2	401043	13	NULL	NULL	0	NULL	donor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In transferase activity assay , a donor with high expression of B had increased B transferase activity in her serum , which suggested that the high-expression phenotype might be under the control of the glycosyltransferase gene .
	manualset3
99212	3	401043	13	NULL	NULL	0	NULL	 high expression of B	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In transferase activity assay , a donor with high expression of B had increased B transferase activity in her serum , which suggested that the high-expression phenotype might be under the control of the glycosyltransferase gene .
	manualset3
99213	4	401043	13	NULL	NULL	0	NULL	B transferase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In transferase activity assay , a donor with high expression of B had increased B transferase activity in her serum , which suggested that the high-expression phenotype might be under the control of the glycosyltransferase gene .
	manualset3
99214	5	401043	13	NULL	NULL	0	NULL	 serum	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In transferase activity assay , a donor with high expression of B had increased B transferase activity in her serum , which suggested that the high-expression phenotype might be under the control of the glycosyltransferase gene .
	manualset3
99215	6	401043	13	NULL	NULL	0	NULL	high-expression phenotype 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In transferase activity assay , a donor with high expression of B had increased B transferase activity in her serum , which suggested that the high-expression phenotype might be under the control of the glycosyltransferase gene .
	manualset3
99216	7	401043	13	NULL	NULL	0	NULL	control 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In transferase activity assay , a donor with high expression of B had increased B transferase activity in her serum , which suggested that the high-expression phenotype might be under the control of the glycosyltransferase gene .
	manualset3
99217	8	401043	13	NULL	NULL	0	NULL	glycosyltransferase gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In transferase activity assay , a donor with high expression of B had increased B transferase activity in her serum , which suggested that the high-expression phenotype might be under the control of the glycosyltransferase gene .
	manualset3
99218	1	401044	13	NULL	NULL	0	NULL	trombophilia screening	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In trombophilia screening only moderate hyperhomocysteinemia ( not related to MTHFR C667T polymorphism ) was found .
	manualset3
99219	2	401044	13	NULL	NULL	0	NULL	moderate hyperhomocysteinemia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In trombophilia screening only moderate hyperhomocysteinemia ( not related to MTHFR C667T polymorphism ) was found .
	manualset3
99220	3	401044	13	NULL	NULL	0	NULL	MTHFR C667T polymorphism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In trombophilia screening only moderate hyperhomocysteinemia ( not related to MTHFR C667T polymorphism ) was found .
	manualset3
99221	1	401045	13	NULL	NULL	0	NULL	 tumor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In tumor cells , expression of iNOS was detected in 35/89 ( 40 % ) cases , while 79/89 ( 89 % ) and 72/89 ( 81 % ) cases showed weak to intense positivity for eNOS and nNOS , respectively .
	manualset3
99222	2	401045	13	NULL	NULL	0	NULL	expression of iNOS	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In tumor cells , expression of iNOS was detected in 35/89 ( 40 % ) cases , while 79/89 ( 89 % ) and 72/89 ( 81 % ) cases showed weak to intense positivity for eNOS and nNOS , respectively .
	manualset3
99223	3	401045	13	NULL	NULL	NULL	NULL	35/89 ( 40 % ) cases	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In tumor cells , expression of iNOS was detected in 35/89 ( 40 % ) cases , while 79/89 ( 89 % ) and 72/89 ( 81 % ) cases showed weak to intense positivity for eNOS and nNOS , respectively .
	manualset3
99224	4	401045	13	NULL	NULL	0	NULL	79/89 ( 89 % ) cases	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In tumor cells , expression of iNOS was detected in 35/89 ( 40 % ) cases , while 79/89 ( 89 % ) and 72/89 ( 81 % ) cases showed weak to intense positivity for eNOS and nNOS , respectively .
	manualset3
99225	5	401045	13	NULL	NULL	0	NULL	 72/89 ( 81 % ) cases	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In tumor cells , expression of iNOS was detected in 35/89 ( 40 % ) cases , while 79/89 ( 89 % ) and 72/89 ( 81 % ) cases showed weak to intense positivity for eNOS and nNOS , respectively .
	manualset3
99226	6	401045	13	NULL	NULL	0	NULL	 intense positivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In tumor cells , expression of iNOS was detected in 35/89 ( 40 % ) cases , while 79/89 ( 89 % ) and 72/89 ( 81 % ) cases showed weak to intense positivity for eNOS and nNOS , respectively .
	manualset3
99227	7	401045	13	NULL	NULL	0	NULL	eNOS	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In tumor cells , expression of iNOS was detected in 35/89 ( 40 % ) cases , while 79/89 ( 89 % ) and 72/89 ( 81 % ) cases showed weak to intense positivity for eNOS and nNOS , respectively .
	manualset3
99228	8	401045	13	NULL	NULL	0	NULL	nNOS	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In tumor cells , expression of iNOS was detected in 35/89 ( 40 % ) cases , while 79/89 ( 89 % ) and 72/89 ( 81 % ) cases showed weak to intense positivity for eNOS and nNOS , respectively .
	manualset3
99229	1	401046	13	NULL	NULL	0	NULL	tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In tumors that retain wild-type p53 , its tumor-suppressor function is often impaired as a result of the deregulation of HDM-2 , which binds to p53 and targets it for proteasomal degradation .
	manualset3
99230	2	401046	13	NULL	NULL	0	NULL	wild-type p53 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In tumors that retain wild-type p53 , its tumor-suppressor function is often impaired as a result of the deregulation of HDM-2 , which binds to p53 and targets it for proteasomal degradation .
	manualset3
99231	3	401046	13	NULL	NULL	0	NULL	tumor-suppressor function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In tumors that retain wild-type p53 , its tumor-suppressor function is often impaired as a result of the deregulation of HDM-2 , which binds to p53 and targets it for proteasomal degradation .
	manualset3
99232	4	401046	13	NULL	NULL	0	NULL	result	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In tumors that retain wild-type p53 , its tumor-suppressor function is often impaired as a result of the deregulation of HDM-2 , which binds to p53 and targets it for proteasomal degradation .
	manualset3
99233	5	401046	13	NULL	NULL	0	NULL	deregulation of HDM-2	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In tumors that retain wild-type p53 , its tumor-suppressor function is often impaired as a result of the deregulation of HDM-2 , which binds to p53 and targets it for proteasomal degradation .
	manualset3
99234	6	401046	13	NULL	NULL	0	NULL	p53	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In tumors that retain wild-type p53 , its tumor-suppressor function is often impaired as a result of the deregulation of HDM-2 , which binds to p53 and targets it for proteasomal degradation .
	manualset3
99235	7	401046	13	NULL	NULL	0	NULL	 targets 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In tumors that retain wild-type p53 , its tumor-suppressor function is often impaired as a result of the deregulation of HDM-2 , which binds to p53 and targets it for proteasomal degradation .
	manualset3
99236	8	401046	13	NULL	NULL	0	NULL	proteasomal degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In tumors that retain wild-type p53 , its tumor-suppressor function is often impaired as a result of the deregulation of HDM-2 , which binds to p53 and targets it for proteasomal degradation .
	manualset3
99237	1	401047	13	NULL	NULL	0	NULL	2	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ( 1 vascular malformation and 1 glioma ) were subtotally removed too , the aneurysm was only given a decompression of increased intracranial pressure , because the patient 's interrupted respiration during the operation .
	manualset3
99238	2	401047	13	NULL	NULL	0	NULL	1 vascular malformation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ( 1 vascular malformation and 1 glioma ) were subtotally removed too , the aneurysm was only given a decompression of increased intracranial pressure , because the patient 's interrupted respiration during the operation .
	manualset3
99239	3	401047	13	NULL	NULL	0	NULL	1 glioma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ( 1 vascular malformation and 1 glioma ) were subtotally removed too , the aneurysm was only given a decompression of increased intracranial pressure , because the patient 's interrupted respiration during the operation .
	manualset3
99240	4	401047	13	NULL	NULL	0	NULL	 aneurysm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ( 1 vascular malformation and 1 glioma ) were subtotally removed too , the aneurysm was only given a decompression of increased intracranial pressure , because the patient 's interrupted respiration during the operation .
	manualset3
99241	5	401047	13	NULL	NULL	0	NULL	 decompression 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ( 1 vascular malformation and 1 glioma ) were subtotally removed too , the aneurysm was only given a decompression of increased intracranial pressure , because the patient 's interrupted respiration during the operation .
	manualset3
99242	6	401047	13	NULL	NULL	0	NULL	intracranial pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ( 1 vascular malformation and 1 glioma ) were subtotally removed too , the aneurysm was only given a decompression of increased intracranial pressure , because the patient 's interrupted respiration during the operation .
	manualset3
99243	7	401047	13	NULL	NULL	0	NULL	 patient 's	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ( 1 vascular malformation and 1 glioma ) were subtotally removed too , the aneurysm was only given a decompression of increased intracranial pressure , because the patient 's interrupted respiration during the operation .
	manualset3
99244	8	401047	13	NULL	NULL	0	NULL	respiration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ( 1 vascular malformation and 1 glioma ) were subtotally removed too , the aneurysm was only given a decompression of increased intracranial pressure , because the patient 's interrupted respiration during the operation .
	manualset3
99245	9	401047	13	NULL	NULL	0	NULL	operation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ( 1 vascular malformation and 1 glioma ) were subtotally removed too , the aneurysm was only given a decompression of increased intracranial pressure , because the patient 's interrupted respiration during the operation .
	manualset3
99246	1	401048	13	NULL	NULL	0	NULL	 type IA	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In type IA , the most important findings are disruption of the network of the intrafollicular dendritic cells , progressive atrophy of the mantle zone as shown with anti-delta antibody , the progressive diminution of the number of CD4 cells first in the germinative centres then in the extrafollicular areas , the progressive increase of CD8 cells first in the germinative centres , the presence of a severe B cells hyperplasia which is polytypic .
	manualset3
99247	2	401048	13	NULL	NULL	0	NULL	important findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In type IA , the most important findings are disruption of the network of the intrafollicular dendritic cells , progressive atrophy of the mantle zone as shown with anti-delta antibody , the progressive diminution of the number of CD4 cells first in the germinative centres then in the extrafollicular areas , the progressive increase of CD8 cells first in the germinative centres , the presence of a severe B cells hyperplasia which is polytypic .
	manualset3
99248	3	401048	13	NULL	NULL	0	NULL	disruption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In type IA , the most important findings are disruption of the network of the intrafollicular dendritic cells , progressive atrophy of the mantle zone as shown with anti-delta antibody , the progressive diminution of the number of CD4 cells first in the germinative centres then in the extrafollicular areas , the progressive increase of CD8 cells first in the germinative centres , the presence of a severe B cells hyperplasia which is polytypic .
	manualset3
99249	4	401048	13	NULL	NULL	0	NULL	network	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In type IA , the most important findings are disruption of the network of the intrafollicular dendritic cells , progressive atrophy of the mantle zone as shown with anti-delta antibody , the progressive diminution of the number of CD4 cells first in the germinative centres then in the extrafollicular areas , the progressive increase of CD8 cells first in the germinative centres , the presence of a severe B cells hyperplasia which is polytypic .
	manualset3
99250	5	401048	13	NULL	NULL	0	NULL	 intrafollicular dendritic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In type IA , the most important findings are disruption of the network of the intrafollicular dendritic cells , progressive atrophy of the mantle zone as shown with anti-delta antibody , the progressive diminution of the number of CD4 cells first in the germinative centres then in the extrafollicular areas , the progressive increase of CD8 cells first in the germinative centres , the presence of a severe B cells hyperplasia which is polytypic .
	manualset3
99251	6	401048	13	NULL	NULL	0	NULL	 progressive atrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In type IA , the most important findings are disruption of the network of the intrafollicular dendritic cells , progressive atrophy of the mantle zone as shown with anti-delta antibody , the progressive diminution of the number of CD4 cells first in the germinative centres then in the extrafollicular areas , the progressive increase of CD8 cells first in the germinative centres , the presence of a severe B cells hyperplasia which is polytypic .
	manualset3
99252	7	401048	13	NULL	NULL	0	NULL	mantle zone	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In type IA , the most important findings are disruption of the network of the intrafollicular dendritic cells , progressive atrophy of the mantle zone as shown with anti-delta antibody , the progressive diminution of the number of CD4 cells first in the germinative centres then in the extrafollicular areas , the progressive increase of CD8 cells first in the germinative centres , the presence of a severe B cells hyperplasia which is polytypic .
	manualset3
99253	8	401048	13	NULL	NULL	0	NULL	anti-delta antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In type IA , the most important findings are disruption of the network of the intrafollicular dendritic cells , progressive atrophy of the mantle zone as shown with anti-delta antibody , the progressive diminution of the number of CD4 cells first in the germinative centres then in the extrafollicular areas , the progressive increase of CD8 cells first in the germinative centres , the presence of a severe B cells hyperplasia which is polytypic .
	manualset3
99254	9	401048	13	NULL	NULL	0	NULL	progressive diminution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In type IA , the most important findings are disruption of the network of the intrafollicular dendritic cells , progressive atrophy of the mantle zone as shown with anti-delta antibody , the progressive diminution of the number of CD4 cells first in the germinative centres then in the extrafollicular areas , the progressive increase of CD8 cells first in the germinative centres , the presence of a severe B cells hyperplasia which is polytypic .
	manualset3
99255	10	401048	13	NULL	NULL	0	NULL	 number of CD4 cells	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In type IA , the most important findings are disruption of the network of the intrafollicular dendritic cells , progressive atrophy of the mantle zone as shown with anti-delta antibody , the progressive diminution of the number of CD4 cells first in the germinative centres then in the extrafollicular areas , the progressive increase of CD8 cells first in the germinative centres , the presence of a severe B cells hyperplasia which is polytypic .
	manualset3
99256	11	401048	13	NULL	NULL	0	NULL	germinative centres	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In type IA , the most important findings are disruption of the network of the intrafollicular dendritic cells , progressive atrophy of the mantle zone as shown with anti-delta antibody , the progressive diminution of the number of CD4 cells first in the germinative centres then in the extrafollicular areas , the progressive increase of CD8 cells first in the germinative centres , the presence of a severe B cells hyperplasia which is polytypic .
	manualset3
99257	12	401048	13	NULL	NULL	0	NULL	extrafollicular areas 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In type IA , the most important findings are disruption of the network of the intrafollicular dendritic cells , progressive atrophy of the mantle zone as shown with anti-delta antibody , the progressive diminution of the number of CD4 cells first in the germinative centres then in the extrafollicular areas , the progressive increase of CD8 cells first in the germinative centres , the presence of a severe B cells hyperplasia which is polytypic .
	manualset3
99258	13	401048	13	NULL	NULL	0	NULL	CD8 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In type IA , the most important findings are disruption of the network of the intrafollicular dendritic cells , progressive atrophy of the mantle zone as shown with anti-delta antibody , the progressive diminution of the number of CD4 cells first in the germinative centres then in the extrafollicular areas , the progressive increase of CD8 cells first in the germinative centres , the presence of a severe B cells hyperplasia which is polytypic .
	manualset3
99259	14	401048	13	NULL	NULL	0	NULL	germinative centres	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In type IA , the most important findings are disruption of the network of the intrafollicular dendritic cells , progressive atrophy of the mantle zone as shown with anti-delta antibody , the progressive diminution of the number of CD4 cells first in the germinative centres then in the extrafollicular areas , the progressive increase of CD8 cells first in the germinative centres , the presence of a severe B cells hyperplasia which is polytypic .
	manualset3
99260	15	401048	13	NULL	NULL	0	NULL	presence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In type IA , the most important findings are disruption of the network of the intrafollicular dendritic cells , progressive atrophy of the mantle zone as shown with anti-delta antibody , the progressive diminution of the number of CD4 cells first in the germinative centres then in the extrafollicular areas , the progressive increase of CD8 cells first in the germinative centres , the presence of a severe B cells hyperplasia which is polytypic .
	manualset3
99261	16	401048	13	NULL	NULL	0	NULL	severe B cells hyperplasia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In type IA , the most important findings are disruption of the network of the intrafollicular dendritic cells , progressive atrophy of the mantle zone as shown with anti-delta antibody , the progressive diminution of the number of CD4 cells first in the germinative centres then in the extrafollicular areas , the progressive increase of CD8 cells first in the germinative centres , the presence of a severe B cells hyperplasia which is polytypic .
	manualset3
99262	1	401049	13	NULL	NULL	0	NULL	type IIb hypercholesterolemia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In type IIb hypercholesterolemia ( 23 patients ) , the association simvastatin-cholestyramine did not appear more effective than simvastatin used alone .
	manualset3
99263	2	401049	13	NULL	NULL	0	NULL	23 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In type IIb hypercholesterolemia ( 23 patients ) , the association simvastatin-cholestyramine did not appear more effective than simvastatin used alone .
	manualset3
99264	3	401049	13	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In type IIb hypercholesterolemia ( 23 patients ) , the association simvastatin-cholestyramine did not appear more effective than simvastatin used alone .
	manualset3
99265	4	401049	13	NULL	NULL	0	NULL	simvastatin-cholestyramine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In type IIb hypercholesterolemia ( 23 patients ) , the association simvastatin-cholestyramine did not appear more effective than simvastatin used alone .
	manualset3
99266	5	401049	13	NULL	NULL	0	NULL	simvastatin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In type IIb hypercholesterolemia ( 23 patients ) , the association simvastatin-cholestyramine did not appear more effective than simvastatin used alone .
	manualset3
99268	1	401050	13	NULL	NULL	0	NULL	univariate survival analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In univariate survival analysis of all invasive ovarian carcinomas , a highly significant association of increased cytoplasmic CD24 expression with shortened patient survival ( mean 98 months versus 37 months , P = 0.0002 , log rank test ) was demonstrated .
	manualset3
99269	2	401050	13	NULL	NULL	0	NULL	invasive ovarian carcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In univariate survival analysis of all invasive ovarian carcinomas , a highly significant association of increased cytoplasmic CD24 expression with shortened patient survival ( mean 98 months versus 37 months , P = 0.0002 , log rank test ) was demonstrated .
	manualset3
99270	3	401050	13	NULL	NULL	0	NULL	 association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In univariate survival analysis of all invasive ovarian carcinomas , a highly significant association of increased cytoplasmic CD24 expression with shortened patient survival ( mean 98 months versus 37 months , P = 0.0002 , log rank test ) was demonstrated .
	manualset3
99271	4	401050	13	NULL	NULL	0	NULL	cytoplasmic CD24 expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In univariate survival analysis of all invasive ovarian carcinomas , a highly significant association of increased cytoplasmic CD24 expression with shortened patient survival ( mean 98 months versus 37 months , P = 0.0002 , log rank test ) was demonstrated .
	manualset3
99272	5	401050	13	NULL	NULL	0	NULL	patient survival 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In univariate survival analysis of all invasive ovarian carcinomas , a highly significant association of increased cytoplasmic CD24 expression with shortened patient survival ( mean 98 months versus 37 months , P = 0.0002 , log rank test ) was demonstrated .
	manualset3
99273	6	401050	13	NULL	NULL	0	NULL	mean 98 months versus 37 months , P = 0.0002 , log rank test	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In univariate survival analysis of all invasive ovarian carcinomas , a highly significant association of increased cytoplasmic CD24 expression with shortened patient survival ( mean 98 months versus 37 months , P = 0.0002 , log rank test ) was demonstrated .
	manualset3
99274	1	401051	13	NULL	NULL	0	NULL	untreated sheep 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In untreated sheep breathing 100 % O2 , survival time was 92.6 + / - 3.4 h and postmortem blood-free lung water to dry lung ratio was 4.4 + / - 0.2 .
	manualset3
99275	2	401051	13	NULL	NULL	0	NULL	breathing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In untreated sheep breathing 100 % O2 , survival time was 92.6 + / - 3.4 h and postmortem blood-free lung water to dry lung ratio was 4.4 + / - 0.2 .
	manualset3
99276	3	401051	13	NULL	NULL	0	NULL	100 % O2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In untreated sheep breathing 100 % O2 , survival time was 92.6 + / - 3.4 h and postmortem blood-free lung water to dry lung ratio was 4.4 + / - 0.2 .
	manualset3
99277	4	401051	13	NULL	NULL	0	NULL	survival time was 92.6 + / - 3.4 h	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In untreated sheep breathing 100 % O2 , survival time was 92.6 + / - 3.4 h and postmortem blood-free lung water to dry lung ratio was 4.4 + / - 0.2 .
	manualset3
99278	5	401051	13	NULL	NULL	NULL	NULL	postmortem	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In untreated sheep breathing 100 % O2 , survival time was 92.6 + / - 3.4 h and postmortem blood-free lung water to dry lung ratio was 4.4 + / - 0.2 .
	manualset3
99279	6	401051	13	NULL	NULL	0	NULL	blood-free lung water to dry lung ratio	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In untreated sheep breathing 100 % O2 , survival time was 92.6 + / - 3.4 h and postmortem blood-free lung water to dry lung ratio was 4.4 + / - 0.2 .
	manualset3
99280	7	401051	13	NULL	NULL	0	NULL	4.4 + / - 0.2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In untreated sheep breathing 100 % O2 , survival time was 92.6 + / - 3.4 h and postmortem blood-free lung water to dry lung ratio was 4.4 + / - 0.2 .
	manualset3
99281	1	401052	13	NULL	NULL	NULL	NULL	exposure	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In utero exposure to valproic acid ( VPA ) during pregnancy is associated with an increased risk of neural tube defects ( NTDs ) .
	manualset3
99282	2	401052	13	NULL	NULL	0	NULL	 valproic acid ( VPA )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In utero exposure to valproic acid ( VPA ) during pregnancy is associated with an increased risk of neural tube defects ( NTDs ) .
	manualset3
99283	3	401052	13	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In utero exposure to valproic acid ( VPA ) during pregnancy is associated with an increased risk of neural tube defects ( NTDs ) .
	manualset3
99284	4	401052	13	NULL	NULL	0	NULL	 risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In utero exposure to valproic acid ( VPA ) during pregnancy is associated with an increased risk of neural tube defects ( NTDs ) .
	manualset3
99285	5	401052	13	NULL	NULL	0	NULL	neural tube defects ( NTDs ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In utero exposure to valproic acid ( VPA ) during pregnancy is associated with an increased risk of neural tube defects ( NTDs ) .
	manualset3
99287	2	401053	13	NULL	NULL	0	NULL	suppression of 2-chimaerin	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In utero suppression of 2-chimaerin arrested neuronal migration at the multipolar stage , leading to accumulation of ectopic neurons in the subcortical region .
	manualset3
99288	3	401053	13	NULL	NULL	0	NULL	neuronal migration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In utero suppression of 2-chimaerin arrested neuronal migration at the multipolar stage , leading to accumulation of ectopic neurons in the subcortical region .
	manualset3
99289	4	401053	13	NULL	NULL	0	NULL	multipolar stage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In utero suppression of 2-chimaerin arrested neuronal migration at the multipolar stage , leading to accumulation of ectopic neurons in the subcortical region .
	manualset3
99290	5	401053	13	NULL	NULL	0	NULL	accumulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In utero suppression of 2-chimaerin arrested neuronal migration at the multipolar stage , leading to accumulation of ectopic neurons in the subcortical region .
	manualset3
99291	6	401053	13	NULL	NULL	0	NULL	ectopic neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In utero suppression of 2-chimaerin arrested neuronal migration at the multipolar stage , leading to accumulation of ectopic neurons in the subcortical region .
	manualset3
99292	7	401053	13	NULL	NULL	0	NULL	subcortical region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In utero suppression of 2-chimaerin arrested neuronal migration at the multipolar stage , leading to accumulation of ectopic neurons in the subcortical region .
	manualset3
99293	1	401054	13	NULL	NULL	0	NULL	rabbits	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In vagotomized rabbits separation of both halves of the medulla by a midline section resulted in a ` desynchronization ' of both phrenic and both efferent vagal inspiratory volleys .
	manualset3
99294	2	401054	13	NULL	NULL	NULL	NULL	separation 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In vagotomized rabbits separation of both halves of the medulla by a midline section resulted in a ` desynchronization ' of both phrenic and both efferent vagal inspiratory volleys .
	manualset3
99295	4	401054	13	NULL	NULL	NULL	NULL	midline section	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In vagotomized rabbits separation of both halves of the medulla by a midline section resulted in a ` desynchronization ' of both phrenic and both efferent vagal inspiratory volleys .
	manualset3
99296	3	401054	13	NULL	NULL	0	NULL	both halves of the medulla	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In vagotomized rabbits separation of both halves of the medulla by a midline section resulted in a ` desynchronization ' of both phrenic and both efferent vagal inspiratory volleys .
	manualset3
99297	5	401054	13	NULL	NULL	0	NULL	` desynchronization '	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In vagotomized rabbits separation of both halves of the medulla by a midline section resulted in a ` desynchronization ' of both phrenic and both efferent vagal inspiratory volleys .
	manualset3
99298	6	401054	13	NULL	NULL	0	NULL	both phrenic vagal inspiratory volleys 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In vagotomized rabbits separation of both halves of the medulla by a midline section resulted in a ` desynchronization ' of both phrenic and both efferent vagal inspiratory volleys .
	manualset3
99299	7	401054	13	NULL	NULL	0	NULL	both efferent vagal inspiratory volleys	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In vagotomized rabbits separation of both halves of the medulla by a midline section resulted in a ` desynchronization ' of both phrenic and both efferent vagal inspiratory volleys .
	manualset3
99300	1	401055	13	NULL	NULL	0	NULL	variants 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In variants without NaCl a hydrolytical activity of plasma membrane H + - ATPase was increased with seedling age and its transport one was changed insignificantly , wherease the response of the weaker vacuolar H + - ATPase was opposite .
	manualset3
99301	2	401055	13	NULL	NULL	0	NULL	NaCl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In variants without NaCl a hydrolytical activity of plasma membrane H + - ATPase was increased with seedling age and its transport one was changed insignificantly , wherease the response of the weaker vacuolar H + - ATPase was opposite .
	manualset3
99302	3	401055	13	NULL	NULL	NULL	NULL	hydrolytical activity 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In variants without NaCl a hydrolytical activity of plasma membrane H + - ATPase was increased with seedling age and its transport one was changed insignificantly , wherease the response of the weaker vacuolar H + - ATPase was opposite .
	manualset3
99303	4	401055	13	NULL	NULL	0	NULL	plasma membrane H + - ATPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In variants without NaCl a hydrolytical activity of plasma membrane H + - ATPase was increased with seedling age and its transport one was changed insignificantly , wherease the response of the weaker vacuolar H + - ATPase was opposite .
	manualset3
99304	5	401055	13	NULL	NULL	0	NULL	 seedling age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In variants without NaCl a hydrolytical activity of plasma membrane H + - ATPase was increased with seedling age and its transport one was changed insignificantly , wherease the response of the weaker vacuolar H + - ATPase was opposite .
	manualset3
99305	6	401055	13	NULL	NULL	NULL	NULL	transport	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In variants without NaCl a hydrolytical activity of plasma membrane H + - ATPase was increased with seedling age and its transport one was changed insignificantly , wherease the response of the weaker vacuolar H + - ATPase was opposite .
	manualset3
99306	7	401055	13	NULL	NULL	NULL	NULL	response	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In variants without NaCl a hydrolytical activity of plasma membrane H + - ATPase was increased with seedling age and its transport one was changed insignificantly , wherease the response of the weaker vacuolar H + - ATPase was opposite .
	manualset3
99307	8	401055	13	NULL	NULL	0	NULL	 vacuolar H + - ATPase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In variants without NaCl a hydrolytical activity of plasma membrane H + - ATPase was increased with seedling age and its transport one was changed insignificantly , wherease the response of the weaker vacuolar H + - ATPase was opposite .
	manualset3
99308	1	401056	13	NULL	NULL	0	NULL	vascular cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In vascular cells , the NADPH oxidase isoforms Nox1 , Nox2 , Nox4 , and Nox5 are expressed , which differ in their activity , response to stimuli , and the type of ROS released .
	manualset3
99309	2	401056	13	NULL	NULL	0	NULL	NADPH oxidase isoforms	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In vascular cells , the NADPH oxidase isoforms Nox1 , Nox2 , Nox4 , and Nox5 are expressed , which differ in their activity , response to stimuli , and the type of ROS released .
	manualset3
99310	3	401056	13	NULL	NULL	0	NULL	Nox1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In vascular cells , the NADPH oxidase isoforms Nox1 , Nox2 , Nox4 , and Nox5 are expressed , which differ in their activity , response to stimuli , and the type of ROS released .
	manualset3
99311	4	401056	13	NULL	NULL	0	NULL	Nox2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In vascular cells , the NADPH oxidase isoforms Nox1 , Nox2 , Nox4 , and Nox5 are expressed , which differ in their activity , response to stimuli , and the type of ROS released .
	manualset3
99312	5	401056	13	NULL	NULL	0	NULL	Nox4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In vascular cells , the NADPH oxidase isoforms Nox1 , Nox2 , Nox4 , and Nox5 are expressed , which differ in their activity , response to stimuli , and the type of ROS released .
	manualset3
99313	6	401056	13	NULL	NULL	0	NULL	Nox5 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In vascular cells , the NADPH oxidase isoforms Nox1 , Nox2 , Nox4 , and Nox5 are expressed , which differ in their activity , response to stimuli , and the type of ROS released .
	manualset3
99314	7	401056	13	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vascular cells , the NADPH oxidase isoforms Nox1 , Nox2 , Nox4 , and Nox5 are expressed , which differ in their activity , response to stimuli , and the type of ROS released .
	manualset3
99315	8	401056	13	NULL	NULL	0	NULL	response to stimuli	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vascular cells , the NADPH oxidase isoforms Nox1 , Nox2 , Nox4 , and Nox5 are expressed , which differ in their activity , response to stimuli , and the type of ROS released .
	manualset3
99316	9	401056	13	NULL	NULL	0	NULL	type of ROS 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In vascular cells , the NADPH oxidase isoforms Nox1 , Nox2 , Nox4 , and Nox5 are expressed , which differ in their activity , response to stimuli , and the type of ROS released .
	manualset3
99317	1	401057	13	NULL	NULL	0	NULL	employers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ) Among the employers in the data base , excess risk factors account for 21 % to 31 % of medical care costs , with a mean of 25 % .
	manualset3
99318	2	401057	13	NULL	NULL	0	NULL	data base	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ) Among the employers in the data base , excess risk factors account for 21 % to 31 % of medical care costs , with a mean of 25 % .
	manualset3
99319	3	401057	13	NULL	NULL	0	NULL	risk factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ) Among the employers in the data base , excess risk factors account for 21 % to 31 % of medical care costs , with a mean of 25 % .
	manualset3
99320	4	401057	13	NULL	NULL	0	NULL	account for 21 % to 31 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ) Among the employers in the data base , excess risk factors account for 21 % to 31 % of medical care costs , with a mean of 25 % .
	manualset3
99321	5	401057	13	NULL	NULL	0	NULL	medical care costs	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ) Among the employers in the data base , excess risk factors account for 21 % to 31 % of medical care costs , with a mean of 25 % .
	manualset3
99322	6	401057	13	NULL	NULL	0	NULL	mean of 25 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ) Among the employers in the data base , excess risk factors account for 21 % to 31 % of medical care costs , with a mean of 25 % .
	manualset3
99323	1	401058	13	NULL	NULL	0	NULL	venous blood samples 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In venous blood samples the serum levels of immunoreactive insulin , C-peptide and glucosamine were determined as well as binding of 125I-insulin to erythrocyte receptors .
	manualset3
99324	2	401058	13	NULL	NULL	0	NULL	serum levels of immunoreactive insulin	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In venous blood samples the serum levels of immunoreactive insulin , C-peptide and glucosamine were determined as well as binding of 125I-insulin to erythrocyte receptors .
	manualset3
99325	3	401058	13	NULL	NULL	0	NULL	serum levels of C-peptide	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In venous blood samples the serum levels of immunoreactive insulin , C-peptide and glucosamine were determined as well as binding of 125I-insulin to erythrocyte receptors .
	manualset3
99326	4	401058	13	NULL	NULL	0	NULL	serum levels of glucosamine	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In venous blood samples the serum levels of immunoreactive insulin , C-peptide and glucosamine were determined as well as binding of 125I-insulin to erythrocyte receptors .
	manualset3
99327	5	401058	13	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In venous blood samples the serum levels of immunoreactive insulin , C-peptide and glucosamine were determined as well as binding of 125I-insulin to erythrocyte receptors .
	manualset3
99328	6	401058	13	NULL	NULL	0	NULL	125I-insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In venous blood samples the serum levels of immunoreactive insulin , C-peptide and glucosamine were determined as well as binding of 125I-insulin to erythrocyte receptors .
	manualset3
99329	7	401058	13	NULL	NULL	0	NULL	erythrocyte receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In venous blood samples the serum levels of immunoreactive insulin , C-peptide and glucosamine were determined as well as binding of 125I-insulin to erythrocyte receptors .
	manualset3
99330	1	401059	13	NULL	NULL	0	NULL	view 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In view of market-driven health-care policies and the move to greater efficiencies within the health-care system , the cost of nursing care is being increasingly scrutinised .
	manualset3
99331	2	401059	13	NULL	NULL	NULL	NULL	health-care policies 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In view of market-driven health-care policies and the move to greater efficiencies within the health-care system , the cost of nursing care is being increasingly scrutinised .
	manualset3
99332	3	401059	13	NULL	NULL	0	NULL	efficiencies 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In view of market-driven health-care policies and the move to greater efficiencies within the health-care system , the cost of nursing care is being increasingly scrutinised .
	manualset3
99333	4	401059	13	NULL	NULL	0	NULL	 health-care system	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In view of market-driven health-care policies and the move to greater efficiencies within the health-care system , the cost of nursing care is being increasingly scrutinised .
	manualset3
99334	5	401059	13	NULL	NULL	0	NULL	cost of nursing care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In view of market-driven health-care policies and the move to greater efficiencies within the health-care system , the cost of nursing care is being increasingly scrutinised .
	manualset3
99335	1	401060	13	NULL	NULL	NULL	NULL	view	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In view of the fact that humoral immunity is enhanced during acute LDV infection , these data provide a positive correlation between increased retention of membrane-bound antigen and enhanced humoral immune responses .
	manualset3
99336	2	401060	13	NULL	NULL	0	NULL	fact	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In view of the fact that humoral immunity is enhanced during acute LDV infection , these data provide a positive correlation between increased retention of membrane-bound antigen and enhanced humoral immune responses .
	manualset3
99337	3	401060	13	NULL	NULL	0	NULL	humoral immunity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In view of the fact that humoral immunity is enhanced during acute LDV infection , these data provide a positive correlation between increased retention of membrane-bound antigen and enhanced humoral immune responses .
	manualset3
99338	4	401060	13	NULL	NULL	0	NULL	acute LDV infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In view of the fact that humoral immunity is enhanced during acute LDV infection , these data provide a positive correlation between increased retention of membrane-bound antigen and enhanced humoral immune responses .
	manualset3
99339	5	401060	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In view of the fact that humoral immunity is enhanced during acute LDV infection , these data provide a positive correlation between increased retention of membrane-bound antigen and enhanced humoral immune responses .
	manualset3
99340	6	401060	13	NULL	NULL	0	NULL	correlation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In view of the fact that humoral immunity is enhanced during acute LDV infection , these data provide a positive correlation between increased retention of membrane-bound antigen and enhanced humoral immune responses .
	manualset3
99341	7	401060	13	NULL	NULL	0	NULL	retention 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In view of the fact that humoral immunity is enhanced during acute LDV infection , these data provide a positive correlation between increased retention of membrane-bound antigen and enhanced humoral immune responses .
	manualset3
99342	8	401060	13	NULL	NULL	0	NULL	membrane-bound antigen	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In view of the fact that humoral immunity is enhanced during acute LDV infection , these data provide a positive correlation between increased retention of membrane-bound antigen and enhanced humoral immune responses .
	manualset3
99343	9	401060	13	NULL	NULL	0	NULL	humoral immune responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In view of the fact that humoral immunity is enhanced during acute LDV infection , these data provide a positive correlation between increased retention of membrane-bound antigen and enhanced humoral immune responses .
	manualset3
99344	1	401061	13	NULL	NULL	0	NULL	view 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In view of the overall disappointing results of this method in achieving a specific diagnosis in ALCAPA , all patients with DCMP with or without suspected fibroelastosis should undergo invasive diagnosis with aortography .
	manualset3
99345	2	401061	13	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In view of the overall disappointing results of this method in achieving a specific diagnosis in ALCAPA , all patients with DCMP with or without suspected fibroelastosis should undergo invasive diagnosis with aortography .
	manualset3
99346	3	401061	13	NULL	NULL	0	NULL	method	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In view of the overall disappointing results of this method in achieving a specific diagnosis in ALCAPA , all patients with DCMP with or without suspected fibroelastosis should undergo invasive diagnosis with aortography .
	manualset3
99347	4	401061	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In view of the overall disappointing results of this method in achieving a specific diagnosis in ALCAPA , all patients with DCMP with or without suspected fibroelastosis should undergo invasive diagnosis with aortography .
	manualset3
99348	5	401061	13	NULL	NULL	0	NULL	ALCAPA	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In view of the overall disappointing results of this method in achieving a specific diagnosis in ALCAPA , all patients with DCMP with or without suspected fibroelastosis should undergo invasive diagnosis with aortography .
	manualset3
99349	6	401061	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In view of the overall disappointing results of this method in achieving a specific diagnosis in ALCAPA , all patients with DCMP with or without suspected fibroelastosis should undergo invasive diagnosis with aortography .
	manualset3
99350	7	401061	13	NULL	NULL	0	NULL	DCMP	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In view of the overall disappointing results of this method in achieving a specific diagnosis in ALCAPA , all patients with DCMP with or without suspected fibroelastosis should undergo invasive diagnosis with aortography .
	manualset3
99351	8	401061	13	NULL	NULL	0	NULL	fibroelastosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In view of the overall disappointing results of this method in achieving a specific diagnosis in ALCAPA , all patients with DCMP with or without suspected fibroelastosis should undergo invasive diagnosis with aortography .
	manualset3
99352	9	401061	13	NULL	NULL	0	NULL	invasive diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In view of the overall disappointing results of this method in achieving a specific diagnosis in ALCAPA , all patients with DCMP with or without suspected fibroelastosis should undergo invasive diagnosis with aortography .
	manualset3
99353	10	401061	13	NULL	NULL	0	NULL	aortography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In view of the overall disappointing results of this method in achieving a specific diagnosis in ALCAPA , all patients with DCMP with or without suspected fibroelastosis should undergo invasive diagnosis with aortography .
	manualset3
99354	1	401062	13	NULL	NULL	0	NULL	view	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In view of this , it is important to ease the patient 's economic burden while pushing for high quality cancer treatment .
	manualset3
99355	2	401062	13	NULL	NULL	0	NULL	patient 's	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In view of this , it is important to ease the patient 's economic burden while pushing for high quality cancer treatment .
	manualset3
99356	3	401062	13	NULL	NULL	0	NULL	economic burden	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In view of this , it is important to ease the patient 's economic burden while pushing for high quality cancer treatment .
	manualset3
99357	4	401062	13	NULL	NULL	0	NULL	high quality cancer treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In view of this , it is important to ease the patient 's economic burden while pushing for high quality cancer treatment .
	manualset3
99358	1	401063	13	NULL	NULL	0	NULL	western Kenya	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In western Kenya , caregivers ' views on the risks and benefits to disclosing children 's HIV status emerged a key theme related to a family 's experience with HIV medications , even for families who had not disclosed the child 's status .
	manualset3
99359	2	401063	13	NULL	NULL	0	NULL	caregivers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In western Kenya , caregivers ' views on the risks and benefits to disclosing children 's HIV status emerged a key theme related to a family 's experience with HIV medications , even for families who had not disclosed the child 's status .
	manualset3
99360	3	401063	13	NULL	NULL	NULL	NULL	views 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In western Kenya , caregivers ' views on the risks and benefits to disclosing children 's HIV status emerged a key theme related to a family 's experience with HIV medications , even for families who had not disclosed the child 's status .
	manualset3
99361	4	401063	13	NULL	NULL	0	NULL	risks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In western Kenya , caregivers ' views on the risks and benefits to disclosing children 's HIV status emerged a key theme related to a family 's experience with HIV medications , even for families who had not disclosed the child 's status .
	manualset3
99362	5	401063	13	NULL	NULL	0	NULL	 benefits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In western Kenya , caregivers ' views on the risks and benefits to disclosing children 's HIV status emerged a key theme related to a family 's experience with HIV medications , even for families who had not disclosed the child 's status .
	manualset3
99363	6	401063	13	NULL	NULL	0	NULL	 children 's	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In western Kenya , caregivers ' views on the risks and benefits to disclosing children 's HIV status emerged a key theme related to a family 's experience with HIV medications , even for families who had not disclosed the child 's status .
	manualset3
99364	7	401063	13	NULL	NULL	0	NULL	HIV status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In western Kenya , caregivers ' views on the risks and benefits to disclosing children 's HIV status emerged a key theme related to a family 's experience with HIV medications , even for families who had not disclosed the child 's status .
	manualset3
99365	8	401063	13	NULL	NULL	0	NULL	key theme	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In western Kenya , caregivers ' views on the risks and benefits to disclosing children 's HIV status emerged a key theme related to a family 's experience with HIV medications , even for families who had not disclosed the child 's status .
	manualset3
99366	9	401063	13	NULL	NULL	0	NULL	family 's experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In western Kenya , caregivers ' views on the risks and benefits to disclosing children 's HIV status emerged a key theme related to a family 's experience with HIV medications , even for families who had not disclosed the child 's status .
	manualset3
99367	10	401063	13	NULL	NULL	0	NULL	 HIV medications	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In western Kenya , caregivers ' views on the risks and benefits to disclosing children 's HIV status emerged a key theme related to a family 's experience with HIV medications , even for families who had not disclosed the child 's status .
	manualset3
99368	11	401063	13	NULL	NULL	0	NULL	families	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In western Kenya , caregivers ' views on the risks and benefits to disclosing children 's HIV status emerged a key theme related to a family 's experience with HIV medications , even for families who had not disclosed the child 's status .
	manualset3
99369	12	401063	13	NULL	NULL	0	NULL	child 's status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In western Kenya , caregivers ' views on the risks and benefits to disclosing children 's HIV status emerged a key theme related to a family 's experience with HIV medications , even for families who had not disclosed the child 's status .
	manualset3
99370	1	401064	13	NULL	NULL	0	NULL	yeast	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In yeast and plants , cation/H ( + ) exchangers are important in shaping cytosolic Ca ( 2 + ) levels involved in signal transduction and providing tolerance to potentially toxic concentrations of cations such as Ca ( 2 + ) , Mn ( 2 + ) and Cd ( 2 + ) .
	manualset3
99371	2	401064	13	NULL	NULL	0	NULL	 plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In yeast and plants , cation/H ( + ) exchangers are important in shaping cytosolic Ca ( 2 + ) levels involved in signal transduction and providing tolerance to potentially toxic concentrations of cations such as Ca ( 2 + ) , Mn ( 2 + ) and Cd ( 2 + ) .
	manualset3
99372	3	401064	13	NULL	NULL	0	NULL	cation/H ( + ) exchangers 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In yeast and plants , cation/H ( + ) exchangers are important in shaping cytosolic Ca ( 2 + ) levels involved in signal transduction and providing tolerance to potentially toxic concentrations of cations such as Ca ( 2 + ) , Mn ( 2 + ) and Cd ( 2 + ) .
	manualset3
99373	4	401064	13	NULL	NULL	0	NULL	cytosolic Ca ( 2 + ) levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In yeast and plants , cation/H ( + ) exchangers are important in shaping cytosolic Ca ( 2 + ) levels involved in signal transduction and providing tolerance to potentially toxic concentrations of cations such as Ca ( 2 + ) , Mn ( 2 + ) and Cd ( 2 + ) .
	manualset3
99374	5	401064	13	NULL	NULL	0	NULL	signal transduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In yeast and plants , cation/H ( + ) exchangers are important in shaping cytosolic Ca ( 2 + ) levels involved in signal transduction and providing tolerance to potentially toxic concentrations of cations such as Ca ( 2 + ) , Mn ( 2 + ) and Cd ( 2 + ) .
	manualset3
99375	6	401064	13	NULL	NULL	0	NULL	tolerance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In yeast and plants , cation/H ( + ) exchangers are important in shaping cytosolic Ca ( 2 + ) levels involved in signal transduction and providing tolerance to potentially toxic concentrations of cations such as Ca ( 2 + ) , Mn ( 2 + ) and Cd ( 2 + ) .
	manualset3
99376	7	401064	13	NULL	NULL	0	NULL	toxic concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In yeast and plants , cation/H ( + ) exchangers are important in shaping cytosolic Ca ( 2 + ) levels involved in signal transduction and providing tolerance to potentially toxic concentrations of cations such as Ca ( 2 + ) , Mn ( 2 + ) and Cd ( 2 + ) .
	manualset3
99377	8	401064	13	NULL	NULL	0	NULL	 cations	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In yeast and plants , cation/H ( + ) exchangers are important in shaping cytosolic Ca ( 2 + ) levels involved in signal transduction and providing tolerance to potentially toxic concentrations of cations such as Ca ( 2 + ) , Mn ( 2 + ) and Cd ( 2 + ) .
	manualset3
99378	9	401064	13	NULL	NULL	0	NULL	Ca ( 2 + ) 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In yeast and plants , cation/H ( + ) exchangers are important in shaping cytosolic Ca ( 2 + ) levels involved in signal transduction and providing tolerance to potentially toxic concentrations of cations such as Ca ( 2 + ) , Mn ( 2 + ) and Cd ( 2 + ) .
	manualset3
99379	10	401064	13	NULL	NULL	0	NULL	Mn ( 2 + )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In yeast and plants , cation/H ( + ) exchangers are important in shaping cytosolic Ca ( 2 + ) levels involved in signal transduction and providing tolerance to potentially toxic concentrations of cations such as Ca ( 2 + ) , Mn ( 2 + ) and Cd ( 2 + ) .
	manualset3
99380	11	401064	13	NULL	NULL	0	NULL	Cd ( 2 + )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In yeast and plants , cation/H ( + ) exchangers are important in shaping cytosolic Ca ( 2 + ) levels involved in signal transduction and providing tolerance to potentially toxic concentrations of cations such as Ca ( 2 + ) , Mn ( 2 + ) and Cd ( 2 + ) .
	manualset3
99381	1	401065	13	NULL	NULL	0	NULL	plasma osmolality	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ) The plasma osmolality just before death varied according to the agents administered and was lowest in the case of 7 % sodium bicarbonate with a level of 441 mOsm/1 .
	manualset3
99382	2	401065	13	NULL	NULL	0	NULL	death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ) The plasma osmolality just before death varied according to the agents administered and was lowest in the case of 7 % sodium bicarbonate with a level of 441 mOsm/1 .
	manualset3
99383	3	401065	13	NULL	NULL	0	NULL	agents 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ) The plasma osmolality just before death varied according to the agents administered and was lowest in the case of 7 % sodium bicarbonate with a level of 441 mOsm/1 .
	manualset3
99384	4	401065	13	NULL	NULL	0	NULL	case 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ) The plasma osmolality just before death varied according to the agents administered and was lowest in the case of 7 % sodium bicarbonate with a level of 441 mOsm/1 .
	manualset3
99385	5	401065	13	NULL	NULL	0	NULL	7 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ) The plasma osmolality just before death varied according to the agents administered and was lowest in the case of 7 % sodium bicarbonate with a level of 441 mOsm/1 .
	manualset3
99386	6	401065	13	NULL	NULL	NULL	NULL	sodium bicarbonate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	2 ) The plasma osmolality just before death varied according to the agents administered and was lowest in the case of 7 % sodium bicarbonate with a level of 441 mOsm/1 .
	manualset3
99387	7	401065	13	NULL	NULL	0	NULL	level of 441 mOsm/1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ) The plasma osmolality just before death varied according to the agents administered and was lowest in the case of 7 % sodium bicarbonate with a level of 441 mOsm/1 .
	manualset3
99388	1	401066	13	NULL	NULL	0	NULL	young normotensive women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In young normotensive women ( 5 without and 5 with chronic oral contraceptives ( = o.c. ) cardiovascular homeostasis was challenged by isoproterenol and ergometer exercise , at normal and at resitricted sodium intake .
	manualset3
99391	2	401066	13	NULL	NULL	0	NULL	 5 without chronic oral contraceptives	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In young normotensive women ( 5 without and 5 with chronic oral contraceptives ( = o.c. ) cardiovascular homeostasis was challenged by isoproterenol and ergometer exercise , at normal and at resitricted sodium intake .
	manualset3
99392	3	401066	13	NULL	NULL	0	NULL	 5 with chronic oral contraceptives	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In young normotensive women ( 5 without and 5 with chronic oral contraceptives ( = o.c. ) cardiovascular homeostasis was challenged by isoproterenol and ergometer exercise , at normal and at resitricted sodium intake .
	manualset3
99393	4	401066	13	NULL	NULL	0	NULL	cardiovascular homeostasis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In young normotensive women ( 5 without and 5 with chronic oral contraceptives ( = o.c. ) cardiovascular homeostasis was challenged by isoproterenol and ergometer exercise , at normal and at resitricted sodium intake .
	manualset3
99395	5	401066	13	NULL	NULL	0	NULL	isoproterenol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In young normotensive women ( 5 without and 5 with chronic oral contraceptives ( = o.c. ) cardiovascular homeostasis was challenged by isoproterenol and ergometer exercise , at normal and at resitricted sodium intake .
	manualset3
99399	6	401066	13	NULL	NULL	0	NULL	ergometer exercise 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In young normotensive women ( 5 without and 5 with chronic oral contraceptives ( = o.c. ) cardiovascular homeostasis was challenged by isoproterenol and ergometer exercise , at normal and at resitricted sodium intake .
	manualset3
99401	7	401066	13	NULL	NULL	0	NULL	normal sodium intake	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	In young normotensive women ( 5 without and 5 with chronic oral contraceptives ( = o.c. ) cardiovascular homeostasis was challenged by isoproterenol and ergometer exercise , at normal and at resitricted sodium intake .
	manualset3
99402	8	401066	13	NULL	NULL	0	NULL	resitricted sodium intake	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	In young normotensive women ( 5 without and 5 with chronic oral contraceptives ( = o.c. ) cardiovascular homeostasis was challenged by isoproterenol and ergometer exercise , at normal and at resitricted sodium intake .
	manualset3
99407	1	401067	13	NULL	NULL	0	NULL	young subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In young subjects , virtually absent TmPO4/GFR responses were found in 3 cases with a relatively low basal TmPO4/GFR ( between 0.92 and 0.98 mmol/liter ) , but these cases showed normal increases in NcAMP .
	manualset3
99414	2	401067	13	NULL	NULL	0	NULL	TmPO4/GFR responses 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In young subjects , virtually absent TmPO4/GFR responses were found in 3 cases with a relatively low basal TmPO4/GFR ( between 0.92 and 0.98 mmol/liter ) , but these cases showed normal increases in NcAMP .
	manualset3
99416	3	401067	13	NULL	NULL	0	NULL	3 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In young subjects , virtually absent TmPO4/GFR responses were found in 3 cases with a relatively low basal TmPO4/GFR ( between 0.92 and 0.98 mmol/liter ) , but these cases showed normal increases in NcAMP .
	manualset3
99419	4	401067	13	NULL	NULL	0	NULL	 low basal TmPO4/GFR	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In young subjects , virtually absent TmPO4/GFR responses were found in 3 cases with a relatively low basal TmPO4/GFR ( between 0.92 and 0.98 mmol/liter ) , but these cases showed normal increases in NcAMP .
	manualset3
99420	5	401067	13	NULL	NULL	0	NULL	between 0.92 and 0.98 mmol/liter	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In young subjects , virtually absent TmPO4/GFR responses were found in 3 cases with a relatively low basal TmPO4/GFR ( between 0.92 and 0.98 mmol/liter ) , but these cases showed normal increases in NcAMP .
	manualset3
99422	6	401067	13	NULL	NULL	0	NULL	cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In young subjects , virtually absent TmPO4/GFR responses were found in 3 cases with a relatively low basal TmPO4/GFR ( between 0.92 and 0.98 mmol/liter ) , but these cases showed normal increases in NcAMP .
	manualset3
99425	7	401067	13	NULL	NULL	NULL	NULL	increases in NcAMP	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In young subjects , virtually absent TmPO4/GFR responses were found in 3 cases with a relatively low basal TmPO4/GFR ( between 0.92 and 0.98 mmol/liter ) , but these cases showed normal increases in NcAMP .
	manualset3
99426	1	401068	13	NULL	NULL	0	NULL	InAs nanowires 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	InAs nanowires are grown epitaxially by catalyst-free metal organic vapor phase epitaxy and are subsequently positioned with a lateral accuracy of less than 1 m using simple adhesion forces between the nanowires and an indium tip .
	manualset3
99427	2	401068	13	NULL	NULL	NULL	NULL	catalyst-free metal 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	InAs nanowires are grown epitaxially by catalyst-free metal organic vapor phase epitaxy and are subsequently positioned with a lateral accuracy of less than 1 m using simple adhesion forces between the nanowires and an indium tip .
	manualset3
99448	3	401068	13	NULL	NULL	0	NULL	organic vapor phase epitaxy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	InAs nanowires are grown epitaxially by catalyst-free metal organic vapor phase epitaxy and are subsequently positioned with a lateral accuracy of less than 1 m using simple adhesion forces between the nanowires and an indium tip .
	manualset3
99449	4	401068	13	NULL	NULL	0	NULL	lateral accuracy 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	InAs nanowires are grown epitaxially by catalyst-free metal organic vapor phase epitaxy and are subsequently positioned with a lateral accuracy of less than 1 m using simple adhesion forces between the nanowires and an indium tip .
	manualset3
99450	5	401068	13	NULL	NULL	0	NULL	less than 1 m	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	InAs nanowires are grown epitaxially by catalyst-free metal organic vapor phase epitaxy and are subsequently positioned with a lateral accuracy of less than 1 m using simple adhesion forces between the nanowires and an indium tip .
	manualset3
99451	6	401068	13	NULL	NULL	0	NULL	adhesion forces	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	InAs nanowires are grown epitaxially by catalyst-free metal organic vapor phase epitaxy and are subsequently positioned with a lateral accuracy of less than 1 m using simple adhesion forces between the nanowires and an indium tip .
	manualset3
99452	7	401068	13	NULL	NULL	0	NULL	nanowires	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	InAs nanowires are grown epitaxially by catalyst-free metal organic vapor phase epitaxy and are subsequently positioned with a lateral accuracy of less than 1 m using simple adhesion forces between the nanowires and an indium tip .
	manualset3
99453	8	401068	13	NULL	NULL	0	NULL	indium tip	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	InAs nanowires are grown epitaxially by catalyst-free metal organic vapor phase epitaxy and are subsequently positioned with a lateral accuracy of less than 1 m using simple adhesion forces between the nanowires and an indium tip .
	manualset3
99458	1	401069	13	NULL	NULL	0	NULL	Inactivation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of Salmonella and Escherichia coli O157 : H7 on lettuce and poultry skin by combinations of levulinic acid and sodium dodecyl sulfate .
	manualset3
99459	2	401069	13	NULL	NULL	0	NULL	Salmonella	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of Salmonella and Escherichia coli O157 : H7 on lettuce and poultry skin by combinations of levulinic acid and sodium dodecyl sulfate .
	manualset3
99460	3	401069	13	NULL	NULL	0	NULL	Escherichia coli O157 : H7	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of Salmonella and Escherichia coli O157 : H7 on lettuce and poultry skin by combinations of levulinic acid and sodium dodecyl sulfate .
	manualset3
99461	4	401069	13	NULL	NULL	0	NULL	lettuce 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of Salmonella and Escherichia coli O157 : H7 on lettuce and poultry skin by combinations of levulinic acid and sodium dodecyl sulfate .
	manualset3
99462	5	401069	13	NULL	NULL	0	NULL	poultry skin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of Salmonella and Escherichia coli O157 : H7 on lettuce and poultry skin by combinations of levulinic acid and sodium dodecyl sulfate .
	manualset3
99463	6	401069	13	NULL	NULL	0	NULL	levulinic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of Salmonella and Escherichia coli O157 : H7 on lettuce and poultry skin by combinations of levulinic acid and sodium dodecyl sulfate .
	manualset3
99464	7	401069	13	NULL	NULL	0	NULL	sodium dodecyl sulfate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of Salmonella and Escherichia coli O157 : H7 on lettuce and poultry skin by combinations of levulinic acid and sodium dodecyl sulfate .
	manualset3
99465	1	401070	13	NULL	NULL	0	NULL	Inactivation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of acid-adapted and nonadapted Escherichia coli O157 : H7 during drying and storage of beef jerky treated with different marinades .
	manualset3
99466	2	401070	13	NULL	NULL	0	NULL	acid-adapted Escherichia coli O157 : H7	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of acid-adapted and nonadapted Escherichia coli O157 : H7 during drying and storage of beef jerky treated with different marinades .
	manualset3
99467	3	401070	13	NULL	NULL	0	NULL	nonadapted Escherichia coli O157 : H7	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of acid-adapted and nonadapted Escherichia coli O157 : H7 during drying and storage of beef jerky treated with different marinades .
	manualset3
99468	4	401070	13	NULL	NULL	0	NULL	drying 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of acid-adapted and nonadapted Escherichia coli O157 : H7 during drying and storage of beef jerky treated with different marinades .
	manualset3
99469	5	401070	13	NULL	NULL	0	NULL	storage 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of acid-adapted and nonadapted Escherichia coli O157 : H7 during drying and storage of beef jerky treated with different marinades .
	manualset3
99470	6	401070	13	NULL	NULL	0	NULL	beef jerky	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of acid-adapted and nonadapted Escherichia coli O157 : H7 during drying and storage of beef jerky treated with different marinades .
	manualset3
99471	7	401070	13	NULL	NULL	0	NULL	marinades	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of acid-adapted and nonadapted Escherichia coli O157 : H7 during drying and storage of beef jerky treated with different marinades .
	manualset3
99472	1	401071	13	NULL	NULL	0	NULL	Inactivation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of the caspase-like site decreased breakdown of model proteins by 12-22 % and of the trypsin-like site by 3-35 % .
	manualset3
99473	2	401071	13	NULL	NULL	0	NULL	caspase-like site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of the caspase-like site decreased breakdown of model proteins by 12-22 % and of the trypsin-like site by 3-35 % .
	manualset3
99474	3	401071	13	NULL	NULL	0	NULL	breakdown	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of the caspase-like site decreased breakdown of model proteins by 12-22 % and of the trypsin-like site by 3-35 % .
	manualset3
99475	4	401071	13	NULL	NULL	0	NULL	model proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of the caspase-like site decreased breakdown of model proteins by 12-22 % and of the trypsin-like site by 3-35 % .
	manualset3
99476	5	401071	13	NULL	NULL	0	NULL	12-22 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of the caspase-like site decreased breakdown of model proteins by 12-22 % and of the trypsin-like site by 3-35 % .
	manualset3
99477	6	401071	13	NULL	NULL	0	NULL	trypsin-like site 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of the caspase-like site decreased breakdown of model proteins by 12-22 % and of the trypsin-like site by 3-35 % .
	manualset3
99478	7	401071	13	NULL	NULL	0	NULL	3-35 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of the caspase-like site decreased breakdown of model proteins by 12-22 % and of the trypsin-like site by 3-35 % .
	manualset3
99479	1	401072	13	NULL	NULL	0	NULL	Inactivation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of the renal microvillus membrane Na + - H + exchanger by histidine-specific reagents .
	manualset3
99480	2	401072	13	NULL	NULL	0	NULL	renal microvillus membrane 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of the renal microvillus membrane Na + - H + exchanger by histidine-specific reagents .
	manualset3
99481	3	401072	13	NULL	NULL	NULL	NULL	Na + - H + exchanger 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Inactivation of the renal microvillus membrane Na + - H + exchanger by histidine-specific reagents .
	manualset3
99482	4	401072	13	NULL	NULL	0	NULL	histidine-specific reagents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of the renal microvillus membrane Na + - H + exchanger by histidine-specific reagents .
	manualset3
99483	1	401073	13	NULL	NULL	0	NULL	2 + / -1.3 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 + / -1.3 and 4.3 + / -1.4 ) , tongue ( 1.8 + / -0.4 and 1.9 + / -0.5 ) and larynx ( 1.5 + / -0.6 and 1.5 + / -0.6 ) remained constant over time ( +0.6 % , +2.8 % , +1.4 % , and -2.4 % ; P & lt ; 0.05 when compared with tumor SUV changes ) .
	manualset3
99484	2	401073	13	NULL	NULL	0	NULL	4.3 + / -1.4	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 + / -1.3 and 4.3 + / -1.4 ) , tongue ( 1.8 + / -0.4 and 1.9 + / -0.5 ) and larynx ( 1.5 + / -0.6 and 1.5 + / -0.6 ) remained constant over time ( +0.6 % , +2.8 % , +1.4 % , and -2.4 % ; P & lt ; 0.05 when compared with tumor SUV changes ) .
	manualset3
99485	3	401073	13	NULL	NULL	0	NULL	 tongue	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	2 + / -1.3 and 4.3 + / -1.4 ) , tongue ( 1.8 + / -0.4 and 1.9 + / -0.5 ) and larynx ( 1.5 + / -0.6 and 1.5 + / -0.6 ) remained constant over time ( +0.6 % , +2.8 % , +1.4 % , and -2.4 % ; P & lt ; 0.05 when compared with tumor SUV changes ) .
	manualset3
99486	4	401073	13	NULL	NULL	0	NULL	1.8 + / -0.4 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 + / -1.3 and 4.3 + / -1.4 ) , tongue ( 1.8 + / -0.4 and 1.9 + / -0.5 ) and larynx ( 1.5 + / -0.6 and 1.5 + / -0.6 ) remained constant over time ( +0.6 % , +2.8 % , +1.4 % , and -2.4 % ; P & lt ; 0.05 when compared with tumor SUV changes ) .
	manualset3
99487	5	401073	13	NULL	NULL	0	NULL	1.9 + / -0.5	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 + / -1.3 and 4.3 + / -1.4 ) , tongue ( 1.8 + / -0.4 and 1.9 + / -0.5 ) and larynx ( 1.5 + / -0.6 and 1.5 + / -0.6 ) remained constant over time ( +0.6 % , +2.8 % , +1.4 % , and -2.4 % ; P & lt ; 0.05 when compared with tumor SUV changes ) .
	manualset3
99488	6	401073	13	NULL	NULL	0	NULL	 larynx 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	2 + / -1.3 and 4.3 + / -1.4 ) , tongue ( 1.8 + / -0.4 and 1.9 + / -0.5 ) and larynx ( 1.5 + / -0.6 and 1.5 + / -0.6 ) remained constant over time ( +0.6 % , +2.8 % , +1.4 % , and -2.4 % ; P & lt ; 0.05 when compared with tumor SUV changes ) .
	manualset3
99489	7	401073	13	NULL	NULL	0	NULL	1.5 + / -0.6	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 + / -1.3 and 4.3 + / -1.4 ) , tongue ( 1.8 + / -0.4 and 1.9 + / -0.5 ) and larynx ( 1.5 + / -0.6 and 1.5 + / -0.6 ) remained constant over time ( +0.6 % , +2.8 % , +1.4 % , and -2.4 % ; P & lt ; 0.05 when compared with tumor SUV changes ) .
	manualset3
99490	8	401073	13	NULL	NULL	0	NULL	1.5 + / -0.6 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 + / -1.3 and 4.3 + / -1.4 ) , tongue ( 1.8 + / -0.4 and 1.9 + / -0.5 ) and larynx ( 1.5 + / -0.6 and 1.5 + / -0.6 ) remained constant over time ( +0.6 % , +2.8 % , +1.4 % , and -2.4 % ; P & lt ; 0.05 when compared with tumor SUV changes ) .
	manualset3
99491	9	401073	13	NULL	NULL	0	NULL	over time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	2 + / -1.3 and 4.3 + / -1.4 ) , tongue ( 1.8 + / -0.4 and 1.9 + / -0.5 ) and larynx ( 1.5 + / -0.6 and 1.5 + / -0.6 ) remained constant over time ( +0.6 % , +2.8 % , +1.4 % , and -2.4 % ; P & lt ; 0.05 when compared with tumor SUV changes ) .
	manualset3
99492	10	401073	13	NULL	NULL	0	NULL	+0.6 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 + / -1.3 and 4.3 + / -1.4 ) , tongue ( 1.8 + / -0.4 and 1.9 + / -0.5 ) and larynx ( 1.5 + / -0.6 and 1.5 + / -0.6 ) remained constant over time ( +0.6 % , +2.8 % , +1.4 % , and -2.4 % ; P & lt ; 0.05 when compared with tumor SUV changes ) .
	manualset3
99493	11	401073	13	NULL	NULL	0	NULL	+2.8 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 + / -1.3 and 4.3 + / -1.4 ) , tongue ( 1.8 + / -0.4 and 1.9 + / -0.5 ) and larynx ( 1.5 + / -0.6 and 1.5 + / -0.6 ) remained constant over time ( +0.6 % , +2.8 % , +1.4 % , and -2.4 % ; P & lt ; 0.05 when compared with tumor SUV changes ) .
	manualset3
99494	12	401073	13	NULL	NULL	0	NULL	+1.4 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 + / -1.3 and 4.3 + / -1.4 ) , tongue ( 1.8 + / -0.4 and 1.9 + / -0.5 ) and larynx ( 1.5 + / -0.6 and 1.5 + / -0.6 ) remained constant over time ( +0.6 % , +2.8 % , +1.4 % , and -2.4 % ; P & lt ; 0.05 when compared with tumor SUV changes ) .
	manualset3
99495	13	401073	13	NULL	NULL	0	NULL	 -2.4 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 + / -1.3 and 4.3 + / -1.4 ) , tongue ( 1.8 + / -0.4 and 1.9 + / -0.5 ) and larynx ( 1.5 + / -0.6 and 1.5 + / -0.6 ) remained constant over time ( +0.6 % , +2.8 % , +1.4 % , and -2.4 % ; P & lt ; 0.05 when compared with tumor SUV changes ) .
	manualset3
99496	14	401073	13	NULL	NULL	0	NULL	P & lt ; 0.05 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 + / -1.3 and 4.3 + / -1.4 ) , tongue ( 1.8 + / -0.4 and 1.9 + / -0.5 ) and larynx ( 1.5 + / -0.6 and 1.5 + / -0.6 ) remained constant over time ( +0.6 % , +2.8 % , +1.4 % , and -2.4 % ; P & lt ; 0.05 when compared with tumor SUV changes ) .
	manualset3
99497	15	401073	13	NULL	NULL	0	NULL	tumor SUV changes	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	2 + / -1.3 and 4.3 + / -1.4 ) , tongue ( 1.8 + / -0.4 and 1.9 + / -0.5 ) and larynx ( 1.5 + / -0.6 and 1.5 + / -0.6 ) remained constant over time ( +0.6 % , +2.8 % , +1.4 % , and -2.4 % ; P & lt ; 0.05 when compared with tumor SUV changes ) .
	manualset3
99498	1	401074	13	NULL	NULL	0	NULL	Inactivation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of transforming functions by irradiation with UV light greatly reduced the ability of EBV to enhance HIV-1 replication in T4 + T cell , suggesting that live virus is needed for enhancement .
	manualset3
99499	2	401074	13	NULL	NULL	0	NULL	 functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of transforming functions by irradiation with UV light greatly reduced the ability of EBV to enhance HIV-1 replication in T4 + T cell , suggesting that live virus is needed for enhancement .
	manualset3
99500	3	401074	13	NULL	NULL	0	NULL	irradiation with UV light	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of transforming functions by irradiation with UV light greatly reduced the ability of EBV to enhance HIV-1 replication in T4 + T cell , suggesting that live virus is needed for enhancement .
	manualset3
99501	4	401074	13	NULL	NULL	0	NULL	ability 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of transforming functions by irradiation with UV light greatly reduced the ability of EBV to enhance HIV-1 replication in T4 + T cell , suggesting that live virus is needed for enhancement .
	manualset3
99502	5	401074	13	NULL	NULL	0	NULL	EBV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of transforming functions by irradiation with UV light greatly reduced the ability of EBV to enhance HIV-1 replication in T4 + T cell , suggesting that live virus is needed for enhancement .
	manualset3
99503	6	401074	13	NULL	NULL	0	NULL	HIV-1 replication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of transforming functions by irradiation with UV light greatly reduced the ability of EBV to enhance HIV-1 replication in T4 + T cell , suggesting that live virus is needed for enhancement .
	manualset3
99504	7	401074	13	NULL	NULL	0	NULL	T4 + T cell 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of transforming functions by irradiation with UV light greatly reduced the ability of EBV to enhance HIV-1 replication in T4 + T cell , suggesting that live virus is needed for enhancement .
	manualset3
99505	8	401074	13	NULL	NULL	0	NULL	virus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of transforming functions by irradiation with UV light greatly reduced the ability of EBV to enhance HIV-1 replication in T4 + T cell , suggesting that live virus is needed for enhancement .
	manualset3
99506	9	401074	13	NULL	NULL	0	NULL	enhancement	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of transforming functions by irradiation with UV light greatly reduced the ability of EBV to enhance HIV-1 replication in T4 + T cell , suggesting that live virus is needed for enhancement .
	manualset3
99507	1	401075	13	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inappropriate activation of p34cdc2 kinase has been shown to occur during apoptosis induced by cytotoxic T-cell derived perforin and fragmentin .
	manualset3
99508	2	401075	13	NULL	NULL	0	NULL	p34cdc2 kinase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Inappropriate activation of p34cdc2 kinase has been shown to occur during apoptosis induced by cytotoxic T-cell derived perforin and fragmentin .
	manualset3
99509	3	401075	13	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inappropriate activation of p34cdc2 kinase has been shown to occur during apoptosis induced by cytotoxic T-cell derived perforin and fragmentin .
	manualset3
99510	4	401075	13	NULL	NULL	0	NULL	cytotoxic T-cell derived perforin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Inappropriate activation of p34cdc2 kinase has been shown to occur during apoptosis induced by cytotoxic T-cell derived perforin and fragmentin .
	manualset3
99511	5	401075	13	NULL	NULL	0	NULL	 fragmentin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Inappropriate activation of p34cdc2 kinase has been shown to occur during apoptosis induced by cytotoxic T-cell derived perforin and fragmentin .
	manualset3
99512	1	401076	13	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inappropriate or excessive activation of the complement system can lead to harmful , potentially life-threatening consequences due to severe inflammatory tissue destruction .
	manualset3
99513	2	401076	13	NULL	NULL	0	NULL	complement system	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Inappropriate or excessive activation of the complement system can lead to harmful , potentially life-threatening consequences due to severe inflammatory tissue destruction .
	manualset3
99514	3	401076	13	NULL	NULL	0	NULL	 life-threatening consequences	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inappropriate or excessive activation of the complement system can lead to harmful , potentially life-threatening consequences due to severe inflammatory tissue destruction .
	manualset3
99515	4	401076	13	NULL	NULL	0	NULL	 inflammatory tissue destruction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inappropriate or excessive activation of the complement system can lead to harmful , potentially life-threatening consequences due to severe inflammatory tissue destruction .
	manualset3
99516	1	401077	13	NULL	NULL	0	NULL	low serum GH	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inappropriately low serum GH in an acromegalic : lysosomal involvement in intracellular hormone degradation .
	manualset3
99517	2	401077	13	NULL	NULL	0	NULL	lysosomal involvement 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inappropriately low serum GH in an acromegalic : lysosomal involvement in intracellular hormone degradation .
	manualset3
99518	3	401077	13	NULL	NULL	0	NULL	intracellular hormone degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inappropriately low serum GH in an acromegalic : lysosomal involvement in intracellular hormone degradation .
	manualset3
99519	1	401078	13	NULL	NULL	0	NULL	Incentive	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Incentive increased the number of correct saccades in the AS task and the performance index in the working memory task .
	manualset3
99520	2	401078	13	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Incentive increased the number of correct saccades in the AS task and the performance index in the working memory task .
	manualset3
99521	3	401078	13	NULL	NULL	0	NULL	correct saccades	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Incentive increased the number of correct saccades in the AS task and the performance index in the working memory task .
	manualset3
99522	4	401078	13	NULL	NULL	0	NULL	AS task	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Incentive increased the number of correct saccades in the AS task and the performance index in the working memory task .
	manualset3
99523	5	401078	13	NULL	NULL	0	NULL	performance index	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Incentive increased the number of correct saccades in the AS task and the performance index in the working memory task .
	manualset3
99524	6	401078	13	NULL	NULL	0	NULL	 memory task 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Incentive increased the number of correct saccades in the AS task and the performance index in the working memory task .
	manualset3
99525	1	401079	13	NULL	NULL	0	NULL	Incidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence , causes and impact on VO2max .
	manualset3
99526	2	401079	13	NULL	NULL	0	NULL	causes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence , causes and impact on VO2max .
	manualset3
99527	3	401079	13	NULL	NULL	0	NULL	impact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence , causes and impact on VO2max .
	manualset3
99528	4	401079	13	NULL	NULL	0	NULL	 VO2max 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence , causes and impact on VO2max .
	manualset3
99529	1	401080	13	NULL	NULL	0	NULL	Incidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence and intensity of postpartum lower abdominal pain .
	manualset3
99530	2	401080	13	NULL	NULL	0	NULL	intensity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence and intensity of postpartum lower abdominal pain .
	manualset3
99531	3	401080	13	NULL	NULL	0	NULL	postpartum lower abdominal pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence and intensity of postpartum lower abdominal pain .
	manualset3
99532	1	401081	13	NULL	NULL	0	NULL	Incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence of asymptomatic coronary thrombosis and plaque disruption : comparison of non-cardiac and cardiac deaths among autopsy cases .
	manualset3
99533	2	401081	13	NULL	NULL	0	NULL	asymptomatic coronary thrombosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence of asymptomatic coronary thrombosis and plaque disruption : comparison of non-cardiac and cardiac deaths among autopsy cases .
	manualset3
99534	3	401081	13	NULL	NULL	0	NULL	plaque disruption	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence of asymptomatic coronary thrombosis and plaque disruption : comparison of non-cardiac and cardiac deaths among autopsy cases .
	manualset3
99535	4	401081	13	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence of asymptomatic coronary thrombosis and plaque disruption : comparison of non-cardiac and cardiac deaths among autopsy cases .
	manualset3
99536	5	401081	13	NULL	NULL	0	NULL	 non-cardiac deaths	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence of asymptomatic coronary thrombosis and plaque disruption : comparison of non-cardiac and cardiac deaths among autopsy cases .
	manualset3
99537	6	401081	13	NULL	NULL	0	NULL	cardiac deaths	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence of asymptomatic coronary thrombosis and plaque disruption : comparison of non-cardiac and cardiac deaths among autopsy cases .
	manualset3
99538	7	401081	13	NULL	NULL	0	NULL	autopsy cases	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence of asymptomatic coronary thrombosis and plaque disruption : comparison of non-cardiac and cardiac deaths among autopsy cases .
	manualset3
99539	1	401082	13	NULL	NULL	0	NULL	2	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , blood samples were collected from 20 prepubertal gilts at 20-min intervals from 0800 to 1200 h and from 2000 to 2400 h until the second day of estrus or for 6 d if the gilt failed to exhibit estrus .
	manualset3
99540	2	401082	13	NULL	NULL	0	NULL	 blood samples	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , blood samples were collected from 20 prepubertal gilts at 20-min intervals from 0800 to 1200 h and from 2000 to 2400 h until the second day of estrus or for 6 d if the gilt failed to exhibit estrus .
	manualset3
99541	3	401082	13	NULL	NULL	0	NULL	20	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , blood samples were collected from 20 prepubertal gilts at 20-min intervals from 0800 to 1200 h and from 2000 to 2400 h until the second day of estrus or for 6 d if the gilt failed to exhibit estrus .
	manualset3
99542	4	401082	13	NULL	NULL	0	NULL	 prepubertal gilts 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , blood samples were collected from 20 prepubertal gilts at 20-min intervals from 0800 to 1200 h and from 2000 to 2400 h until the second day of estrus or for 6 d if the gilt failed to exhibit estrus .
	manualset3
99543	5	401082	13	NULL	NULL	NULL	NULL	20-min intervals	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	2 , blood samples were collected from 20 prepubertal gilts at 20-min intervals from 0800 to 1200 h and from 2000 to 2400 h until the second day of estrus or for 6 d if the gilt failed to exhibit estrus .
	manualset3
99544	6	401082	13	NULL	NULL	NULL	NULL	0800 to 1200 h	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	2 , blood samples were collected from 20 prepubertal gilts at 20-min intervals from 0800 to 1200 h and from 2000 to 2400 h until the second day of estrus or for 6 d if the gilt failed to exhibit estrus .
	manualset3
99545	7	401082	13	NULL	NULL	0	NULL	2000 to 2400 h 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , blood samples were collected from 20 prepubertal gilts at 20-min intervals from 0800 to 1200 h and from 2000 to 2400 h until the second day of estrus or for 6 d if the gilt failed to exhibit estrus .
	manualset3
99546	8	401082	13	NULL	NULL	0	NULL	second day 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , blood samples were collected from 20 prepubertal gilts at 20-min intervals from 0800 to 1200 h and from 2000 to 2400 h until the second day of estrus or for 6 d if the gilt failed to exhibit estrus .
	manualset3
99547	9	401082	13	NULL	NULL	0	NULL	estrus	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , blood samples were collected from 20 prepubertal gilts at 20-min intervals from 0800 to 1200 h and from 2000 to 2400 h until the second day of estrus or for 6 d if the gilt failed to exhibit estrus .
	manualset3
99548	10	401082	13	NULL	NULL	0	NULL	6 d 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , blood samples were collected from 20 prepubertal gilts at 20-min intervals from 0800 to 1200 h and from 2000 to 2400 h until the second day of estrus or for 6 d if the gilt failed to exhibit estrus .
	manualset3
99549	11	401082	13	NULL	NULL	0	NULL	 gilt	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , blood samples were collected from 20 prepubertal gilts at 20-min intervals from 0800 to 1200 h and from 2000 to 2400 h until the second day of estrus or for 6 d if the gilt failed to exhibit estrus .
	manualset3
99550	12	401082	13	NULL	NULL	0	NULL	estrus	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , blood samples were collected from 20 prepubertal gilts at 20-min intervals from 0800 to 1200 h and from 2000 to 2400 h until the second day of estrus or for 6 d if the gilt failed to exhibit estrus .
	manualset3
99551	1	401083	13	NULL	NULL	0	NULL	Incidence	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence of epidural catheter replacement in parturients : a retrospective chart review .
	manualset3
99552	2	401083	13	NULL	NULL	NULL	NULL	epidural catheter replacement 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Incidence of epidural catheter replacement in parturients : a retrospective chart review .
	manualset3
99553	3	401083	13	NULL	NULL	0	NULL	parturients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence of epidural catheter replacement in parturients : a retrospective chart review .
	manualset3
99554	4	401083	13	NULL	NULL	0	NULL	retrospective chart review	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence of epidural catheter replacement in parturients : a retrospective chart review .
	manualset3
99555	1	401084	13	NULL	NULL	0	NULL	Incidence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence of host site complications in periocular full thickness skin grafts .
	manualset3
99556	2	401084	13	NULL	NULL	0	NULL	host site complications 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence of host site complications in periocular full thickness skin grafts .
	manualset3
99557	3	401084	13	NULL	NULL	0	NULL	skin grafts 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence of host site complications in periocular full thickness skin grafts .
	manualset3
99558	1	401085	13	NULL	NULL	0	NULL	Incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence of pressure ulcers in intensive care unit patients at risk according to the Waterlow scale and factors influencing the development of pressure ulcers .
	manualset3
99559	2	401085	13	NULL	NULL	0	NULL	pressure ulcers	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence of pressure ulcers in intensive care unit patients at risk according to the Waterlow scale and factors influencing the development of pressure ulcers .
	manualset3
99560	3	401085	13	NULL	NULL	0	NULL	intensive care unit 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence of pressure ulcers in intensive care unit patients at risk according to the Waterlow scale and factors influencing the development of pressure ulcers .
	manualset3
99561	4	401085	13	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence of pressure ulcers in intensive care unit patients at risk according to the Waterlow scale and factors influencing the development of pressure ulcers .
	manualset3
99562	5	401085	13	NULL	NULL	0	NULL	risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence of pressure ulcers in intensive care unit patients at risk according to the Waterlow scale and factors influencing the development of pressure ulcers .
	manualset3
99563	6	401085	13	NULL	NULL	0	NULL	Waterlow scale	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence of pressure ulcers in intensive care unit patients at risk according to the Waterlow scale and factors influencing the development of pressure ulcers .
	manualset3
99564	7	401085	13	NULL	NULL	0	NULL	 factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence of pressure ulcers in intensive care unit patients at risk according to the Waterlow scale and factors influencing the development of pressure ulcers .
	manualset3
99565	8	401085	13	NULL	NULL	NULL	NULL	development 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Incidence of pressure ulcers in intensive care unit patients at risk according to the Waterlow scale and factors influencing the development of pressure ulcers .
	manualset3
99566	9	401085	13	NULL	NULL	0	NULL	pressure ulcers	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence of pressure ulcers in intensive care unit patients at risk according to the Waterlow scale and factors influencing the development of pressure ulcers .
	manualset3
99567	1	401086	13	NULL	NULL	0	NULL	Incidence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence of sensory integrative dysfunction among children with orofacial cleft .
	manualset3
99568	2	401086	13	NULL	NULL	0	NULL	 sensory integrative dysfunction 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence of sensory integrative dysfunction among children with orofacial cleft .
	manualset3
99569	3	401086	13	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence of sensory integrative dysfunction among children with orofacial cleft .
	manualset3
99570	4	401086	13	NULL	NULL	0	NULL	orofacial cleft	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence of sensory integrative dysfunction among children with orofacial cleft .
	manualset3
99571	1	401087	13	NULL	NULL	0	NULL	Incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence of thrombotic complications in patients with hematological malignancies with central venous catheters : a prospective multicentre study .
	manualset3
99572	2	401087	13	NULL	NULL	0	NULL	thrombotic complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence of thrombotic complications in patients with hematological malignancies with central venous catheters : a prospective multicentre study .
	manualset3
99573	3	401087	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence of thrombotic complications in patients with hematological malignancies with central venous catheters : a prospective multicentre study .
	manualset3
99574	4	401087	13	NULL	NULL	0	NULL	hematological malignancies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence of thrombotic complications in patients with hematological malignancies with central venous catheters : a prospective multicentre study .
	manualset3
99575	5	401087	13	NULL	NULL	0	NULL	central venous catheters 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidence of thrombotic complications in patients with hematological malignancies with central venous catheters : a prospective multicentre study .
	manualset3
99576	6	401087	13	NULL	NULL	NULL	NULL	multicentre study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Incidence of thrombotic complications in patients with hematological malignancies with central venous catheters : a prospective multicentre study .
	manualset3
99577	1	401088	13	NULL	NULL	0	NULL	Incidences	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidences of hepatocellular carcinomas and hepatocellular adenomas in the females fed diets containing biphenyl were significantly increased in a dose-related manner , and exceeded a range of the historical control data in the Japan Bioassay Research Center .
	manualset3
99578	2	401088	13	NULL	NULL	0	NULL	hepatocellular carcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidences of hepatocellular carcinomas and hepatocellular adenomas in the females fed diets containing biphenyl were significantly increased in a dose-related manner , and exceeded a range of the historical control data in the Japan Bioassay Research Center .
	manualset3
99579	3	401088	13	NULL	NULL	0	NULL	hepatocellular adenomas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidences of hepatocellular carcinomas and hepatocellular adenomas in the females fed diets containing biphenyl were significantly increased in a dose-related manner , and exceeded a range of the historical control data in the Japan Bioassay Research Center .
	manualset3
99580	4	401088	13	NULL	NULL	0	NULL	females	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidences of hepatocellular carcinomas and hepatocellular adenomas in the females fed diets containing biphenyl were significantly increased in a dose-related manner , and exceeded a range of the historical control data in the Japan Bioassay Research Center .
	manualset3
99581	5	401088	13	NULL	NULL	NULL	NULL	diets	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Incidences of hepatocellular carcinomas and hepatocellular adenomas in the females fed diets containing biphenyl were significantly increased in a dose-related manner , and exceeded a range of the historical control data in the Japan Bioassay Research Center .
	manualset3
99582	6	401088	13	NULL	NULL	0	NULL	biphenyl 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidences of hepatocellular carcinomas and hepatocellular adenomas in the females fed diets containing biphenyl were significantly increased in a dose-related manner , and exceeded a range of the historical control data in the Japan Bioassay Research Center .
	manualset3
99583	7	401088	13	NULL	NULL	0	NULL	dose-related manner	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidences of hepatocellular carcinomas and hepatocellular adenomas in the females fed diets containing biphenyl were significantly increased in a dose-related manner , and exceeded a range of the historical control data in the Japan Bioassay Research Center .
	manualset3
99584	8	401088	13	NULL	NULL	0	NULL	range 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidences of hepatocellular carcinomas and hepatocellular adenomas in the females fed diets containing biphenyl were significantly increased in a dose-related manner , and exceeded a range of the historical control data in the Japan Bioassay Research Center .
	manualset3
99585	9	401088	13	NULL	NULL	0	NULL	 historical control data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidences of hepatocellular carcinomas and hepatocellular adenomas in the females fed diets containing biphenyl were significantly increased in a dose-related manner , and exceeded a range of the historical control data in the Japan Bioassay Research Center .
	manualset3
99586	10	401088	13	NULL	NULL	0	NULL	Japan Bioassay Research Center	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidences of hepatocellular carcinomas and hepatocellular adenomas in the females fed diets containing biphenyl were significantly increased in a dose-related manner , and exceeded a range of the historical control data in the Japan Bioassay Research Center .
	manualset3
99587	1	401089	13	NULL	NULL	0	NULL	listings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Included are listings of the top 25 congressional recipients , the top 25 Senate recipients , and the top 50 House recipients of contributions from medical-industry PACs ; medical-industry PAC contributions to members of the four key congressional committees and to the congressional leadership ; top congressional recipients of contributions from medical professionals ' PACs , including the American Medical Association , from health insurance PACs from pharmaceutical PACs , and from hospitals and care-provider PACs ; and the top medical-industry PACs .
	manualset3
99588	2	401089	13	NULL	NULL	0	NULL	top 25 congressional recipients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Included are listings of the top 25 congressional recipients , the top 25 Senate recipients , and the top 50 House recipients of contributions from medical-industry PACs ; medical-industry PAC contributions to members of the four key congressional committees and to the congressional leadership ; top congressional recipients of contributions from medical professionals ' PACs , including the American Medical Association , from health insurance PACs from pharmaceutical PACs , and from hospitals and care-provider PACs ; and the top medical-industry PACs .
	manualset3
99589	3	401089	13	NULL	NULL	0	NULL	top 25 Senate recipients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Included are listings of the top 25 congressional recipients , the top 25 Senate recipients , and the top 50 House recipients of contributions from medical-industry PACs ; medical-industry PAC contributions to members of the four key congressional committees and to the congressional leadership ; top congressional recipients of contributions from medical professionals ' PACs , including the American Medical Association , from health insurance PACs from pharmaceutical PACs , and from hospitals and care-provider PACs ; and the top medical-industry PACs .
	manualset3
99590	4	401089	13	NULL	NULL	0	NULL	top 50 House recipients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Included are listings of the top 25 congressional recipients , the top 25 Senate recipients , and the top 50 House recipients of contributions from medical-industry PACs ; medical-industry PAC contributions to members of the four key congressional committees and to the congressional leadership ; top congressional recipients of contributions from medical professionals ' PACs , including the American Medical Association , from health insurance PACs from pharmaceutical PACs , and from hospitals and care-provider PACs ; and the top medical-industry PACs .
	manualset3
99591	5	401089	13	NULL	NULL	0	NULL	contributions 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Included are listings of the top 25 congressional recipients , the top 25 Senate recipients , and the top 50 House recipients of contributions from medical-industry PACs ; medical-industry PAC contributions to members of the four key congressional committees and to the congressional leadership ; top congressional recipients of contributions from medical professionals ' PACs , including the American Medical Association , from health insurance PACs from pharmaceutical PACs , and from hospitals and care-provider PACs ; and the top medical-industry PACs .
	manualset3
99592	6	401089	13	NULL	NULL	NULL	NULL	medical-industry PACs	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Included are listings of the top 25 congressional recipients , the top 25 Senate recipients , and the top 50 House recipients of contributions from medical-industry PACs ; medical-industry PAC contributions to members of the four key congressional committees and to the congressional leadership ; top congressional recipients of contributions from medical professionals ' PACs , including the American Medical Association , from health insurance PACs from pharmaceutical PACs , and from hospitals and care-provider PACs ; and the top medical-industry PACs .
	manualset3
99593	7	401089	13	NULL	NULL	0	NULL	 medical-industry PAC contributions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Included are listings of the top 25 congressional recipients , the top 25 Senate recipients , and the top 50 House recipients of contributions from medical-industry PACs ; medical-industry PAC contributions to members of the four key congressional committees and to the congressional leadership ; top congressional recipients of contributions from medical professionals ' PACs , including the American Medical Association , from health insurance PACs from pharmaceutical PACs , and from hospitals and care-provider PACs ; and the top medical-industry PACs .
	manualset3
99594	8	401089	13	NULL	NULL	0	NULL	members	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Included are listings of the top 25 congressional recipients , the top 25 Senate recipients , and the top 50 House recipients of contributions from medical-industry PACs ; medical-industry PAC contributions to members of the four key congressional committees and to the congressional leadership ; top congressional recipients of contributions from medical professionals ' PACs , including the American Medical Association , from health insurance PACs from pharmaceutical PACs , and from hospitals and care-provider PACs ; and the top medical-industry PACs .
	manualset3
99595	9	401089	13	NULL	NULL	0	NULL	four key congressional committees	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Included are listings of the top 25 congressional recipients , the top 25 Senate recipients , and the top 50 House recipients of contributions from medical-industry PACs ; medical-industry PAC contributions to members of the four key congressional committees and to the congressional leadership ; top congressional recipients of contributions from medical professionals ' PACs , including the American Medical Association , from health insurance PACs from pharmaceutical PACs , and from hospitals and care-provider PACs ; and the top medical-industry PACs .
	manualset3
99596	10	401089	13	NULL	NULL	0	NULL	congressional leadership	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Included are listings of the top 25 congressional recipients , the top 25 Senate recipients , and the top 50 House recipients of contributions from medical-industry PACs ; medical-industry PAC contributions to members of the four key congressional committees and to the congressional leadership ; top congressional recipients of contributions from medical professionals ' PACs , including the American Medical Association , from health insurance PACs from pharmaceutical PACs , and from hospitals and care-provider PACs ; and the top medical-industry PACs .
	manualset3
99597	11	401089	13	NULL	NULL	0	NULL	top congressional recipients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Included are listings of the top 25 congressional recipients , the top 25 Senate recipients , and the top 50 House recipients of contributions from medical-industry PACs ; medical-industry PAC contributions to members of the four key congressional committees and to the congressional leadership ; top congressional recipients of contributions from medical professionals ' PACs , including the American Medical Association , from health insurance PACs from pharmaceutical PACs , and from hospitals and care-provider PACs ; and the top medical-industry PACs .
	manualset3
99598	12	401089	13	NULL	NULL	0	NULL	contributions 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Included are listings of the top 25 congressional recipients , the top 25 Senate recipients , and the top 50 House recipients of contributions from medical-industry PACs ; medical-industry PAC contributions to members of the four key congressional committees and to the congressional leadership ; top congressional recipients of contributions from medical professionals ' PACs , including the American Medical Association , from health insurance PACs from pharmaceutical PACs , and from hospitals and care-provider PACs ; and the top medical-industry PACs .
	manualset3
99599	13	401089	13	NULL	NULL	0	NULL	medical professionals ' PACs	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Included are listings of the top 25 congressional recipients , the top 25 Senate recipients , and the top 50 House recipients of contributions from medical-industry PACs ; medical-industry PAC contributions to members of the four key congressional committees and to the congressional leadership ; top congressional recipients of contributions from medical professionals ' PACs , including the American Medical Association , from health insurance PACs from pharmaceutical PACs , and from hospitals and care-provider PACs ; and the top medical-industry PACs .
	manualset3
99600	14	401089	13	NULL	NULL	0	NULL	American Medical Association	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Included are listings of the top 25 congressional recipients , the top 25 Senate recipients , and the top 50 House recipients of contributions from medical-industry PACs ; medical-industry PAC contributions to members of the four key congressional committees and to the congressional leadership ; top congressional recipients of contributions from medical professionals ' PACs , including the American Medical Association , from health insurance PACs from pharmaceutical PACs , and from hospitals and care-provider PACs ; and the top medical-industry PACs .
	manualset3
99601	15	401089	13	NULL	NULL	0	NULL	health insurance PACs	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Included are listings of the top 25 congressional recipients , the top 25 Senate recipients , and the top 50 House recipients of contributions from medical-industry PACs ; medical-industry PAC contributions to members of the four key congressional committees and to the congressional leadership ; top congressional recipients of contributions from medical professionals ' PACs , including the American Medical Association , from health insurance PACs from pharmaceutical PACs , and from hospitals and care-provider PACs ; and the top medical-industry PACs .
	manualset3
99603	17	401089	13	NULL	NULL	0	NULL	hospitals	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Included are listings of the top 25 congressional recipients , the top 25 Senate recipients , and the top 50 House recipients of contributions from medical-industry PACs ; medical-industry PAC contributions to members of the four key congressional committees and to the congressional leadership ; top congressional recipients of contributions from medical professionals ' PACs , including the American Medical Association , from health insurance PACs from pharmaceutical PACs , and from hospitals and care-provider PACs ; and the top medical-industry PACs .
	manualset3
99604	18	401089	13	NULL	NULL	0	NULL	care-provider PACs	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Included are listings of the top 25 congressional recipients , the top 25 Senate recipients , and the top 50 House recipients of contributions from medical-industry PACs ; medical-industry PAC contributions to members of the four key congressional committees and to the congressional leadership ; top congressional recipients of contributions from medical professionals ' PACs , including the American Medical Association , from health insurance PACs from pharmaceutical PACs , and from hospitals and care-provider PACs ; and the top medical-industry PACs .
	manualset3
99605	19	401089	13	NULL	NULL	0	NULL	top medical-industry PACs	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Included are listings of the top 25 congressional recipients , the top 25 Senate recipients , and the top 50 House recipients of contributions from medical-industry PACs ; medical-industry PAC contributions to members of the four key congressional committees and to the congressional leadership ; top congressional recipients of contributions from medical professionals ' PACs , including the American Medical Association , from health insurance PACs from pharmaceutical PACs , and from hospitals and care-provider PACs ; and the top medical-industry PACs .
	manualset3
99602	1	401090	13	NULL	NULL	NULL	NULL	2	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	2 , linear effects on ADG ( 713 , 750 , 800 , 796 , and 785 g/d ; P = 0.05 ) and G : F ( P = 0.07 ) were observed with increasing SID Val : Lys , characterized by improvements to a ratio of 65 % and a plateau thereafter .
	manualset3
99606	2	401090	13	NULL	NULL	0	NULL	linear effects	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , linear effects on ADG ( 713 , 750 , 800 , 796 , and 785 g/d ; P = 0.05 ) and G : F ( P = 0.07 ) were observed with increasing SID Val : Lys , characterized by improvements to a ratio of 65 % and a plateau thereafter .
	manualset3
99607	3	401090	13	NULL	NULL	0	NULL	ADG	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , linear effects on ADG ( 713 , 750 , 800 , 796 , and 785 g/d ; P = 0.05 ) and G : F ( P = 0.07 ) were observed with increasing SID Val : Lys , characterized by improvements to a ratio of 65 % and a plateau thereafter .
	manualset3
99608	4	401090	13	NULL	NULL	0	NULL	713 g/d	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , linear effects on ADG ( 713 , 750 , 800 , 796 , and 785 g/d ; P = 0.05 ) and G : F ( P = 0.07 ) were observed with increasing SID Val : Lys , characterized by improvements to a ratio of 65 % and a plateau thereafter .
	manualset3
99609	5	401090	13	NULL	NULL	0	NULL	750 g/d	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , linear effects on ADG ( 713 , 750 , 800 , 796 , and 785 g/d ; P = 0.05 ) and G : F ( P = 0.07 ) were observed with increasing SID Val : Lys , characterized by improvements to a ratio of 65 % and a plateau thereafter .
	manualset3
99610	6	401090	13	NULL	NULL	0	NULL	 800 g/d	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , linear effects on ADG ( 713 , 750 , 800 , 796 , and 785 g/d ; P = 0.05 ) and G : F ( P = 0.07 ) were observed with increasing SID Val : Lys , characterized by improvements to a ratio of 65 % and a plateau thereafter .
	manualset3
99611	7	401090	13	NULL	NULL	0	NULL	796 g/d	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , linear effects on ADG ( 713 , 750 , 800 , 796 , and 785 g/d ; P = 0.05 ) and G : F ( P = 0.07 ) were observed with increasing SID Val : Lys , characterized by improvements to a ratio of 65 % and a plateau thereafter .
	manualset3
99612	8	401090	13	NULL	NULL	0	NULL	785 g/d	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , linear effects on ADG ( 713 , 750 , 800 , 796 , and 785 g/d ; P = 0.05 ) and G : F ( P = 0.07 ) were observed with increasing SID Val : Lys , characterized by improvements to a ratio of 65 % and a plateau thereafter .
	manualset3
99613	9	401090	13	NULL	NULL	0	NULL	P = 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , linear effects on ADG ( 713 , 750 , 800 , 796 , and 785 g/d ; P = 0.05 ) and G : F ( P = 0.07 ) were observed with increasing SID Val : Lys , characterized by improvements to a ratio of 65 % and a plateau thereafter .
	manualset3
99614	10	401090	13	NULL	NULL	0	NULL	G : F ( P = 0.07 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , linear effects on ADG ( 713 , 750 , 800 , 796 , and 785 g/d ; P = 0.05 ) and G : F ( P = 0.07 ) were observed with increasing SID Val : Lys , characterized by improvements to a ratio of 65 % and a plateau thereafter .
	manualset3
99615	11	401090	13	NULL	NULL	0	NULL	SID Val : Lys	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , linear effects on ADG ( 713 , 750 , 800 , 796 , and 785 g/d ; P = 0.05 ) and G : F ( P = 0.07 ) were observed with increasing SID Val : Lys , characterized by improvements to a ratio of 65 % and a plateau thereafter .
	manualset3
99616	12	401090	13	NULL	NULL	0	NULL	improvements 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , linear effects on ADG ( 713 , 750 , 800 , 796 , and 785 g/d ; P = 0.05 ) and G : F ( P = 0.07 ) were observed with increasing SID Val : Lys , characterized by improvements to a ratio of 65 % and a plateau thereafter .
	manualset3
99617	13	401090	13	NULL	NULL	0	NULL	ratio of 65 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , linear effects on ADG ( 713 , 750 , 800 , 796 , and 785 g/d ; P = 0.05 ) and G : F ( P = 0.07 ) were observed with increasing SID Val : Lys , characterized by improvements to a ratio of 65 % and a plateau thereafter .
	manualset3
99618	14	401090	13	NULL	NULL	0	NULL	plateau 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 , linear effects on ADG ( 713 , 750 , 800 , 796 , and 785 g/d ; P = 0.05 ) and G : F ( P = 0.07 ) were observed with increasing SID Val : Lys , characterized by improvements to a ratio of 65 % and a plateau thereafter .
	manualset3
99619	1	401091	13	NULL	NULL	0	NULL	p55 accessory subunit 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Including the p55 accessory subunit , which confers processivity to the pol gamma catalytic subunit , decreases frameshift and base substitution fidelity .
	manualset3
99620	2	401091	13	NULL	NULL	0	NULL	processivity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Including the p55 accessory subunit , which confers processivity to the pol gamma catalytic subunit , decreases frameshift and base substitution fidelity .
	manualset3
99621	3	401091	13	NULL	NULL	0	NULL	pol gamma catalytic subunit	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Including the p55 accessory subunit , which confers processivity to the pol gamma catalytic subunit , decreases frameshift and base substitution fidelity .
	manualset3
99622	4	401091	13	NULL	NULL	0	NULL	frameshift 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Including the p55 accessory subunit , which confers processivity to the pol gamma catalytic subunit , decreases frameshift and base substitution fidelity .
	manualset3
99623	5	401091	13	NULL	NULL	0	NULL	base substitution fidelity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Including the p55 accessory subunit , which confers processivity to the pol gamma catalytic subunit , decreases frameshift and base substitution fidelity .
	manualset3
99624	1	401092	13	NULL	NULL	0	NULL	Inclusion criteria	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inclusion criteria were age & lt ; 15 years at time of presentation who were resident in the eastern part of the country and who diagnosed with inflammatory bowel disease .
	manualset3
99625	2	401092	13	NULL	NULL	0	NULL	age & lt	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Inclusion criteria were age & lt ; 15 years at time of presentation who were resident in the eastern part of the country and who diagnosed with inflammatory bowel disease .
	manualset3
99626	3	401092	13	NULL	NULL	NULL	NULL	15 years	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Inclusion criteria were age & lt ; 15 years at time of presentation who were resident in the eastern part of the country and who diagnosed with inflammatory bowel disease .
	manualset3
99627	4	401092	13	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Inclusion criteria were age & lt ; 15 years at time of presentation who were resident in the eastern part of the country and who diagnosed with inflammatory bowel disease .
	manualset3
99628	5	401092	13	NULL	NULL	0	NULL	presentation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inclusion criteria were age & lt ; 15 years at time of presentation who were resident in the eastern part of the country and who diagnosed with inflammatory bowel disease .
	manualset3
99629	6	401092	13	NULL	NULL	0	NULL	 resident	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Inclusion criteria were age & lt ; 15 years at time of presentation who were resident in the eastern part of the country and who diagnosed with inflammatory bowel disease .
	manualset3
99630	7	401092	13	NULL	NULL	0	NULL	eastern part of the country 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Inclusion criteria were age & lt ; 15 years at time of presentation who were resident in the eastern part of the country and who diagnosed with inflammatory bowel disease .
	manualset3
99631	8	401092	13	NULL	NULL	0	NULL	inflammatory bowel disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Inclusion criteria were age & lt ; 15 years at time of presentation who were resident in the eastern part of the country and who diagnosed with inflammatory bowel disease .
	manualset3
99632	1	401093	13	NULL	NULL	NULL	NULL	Incorporation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Incorporation of 5-bromodeoxyuridine into DNA in newborn rat tissues .
	manualset3
99633	2	401093	13	NULL	NULL	0	NULL	 5-bromodeoxyuridine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of 5-bromodeoxyuridine into DNA in newborn rat tissues .
	manualset3
99634	3	401093	13	NULL	NULL	0	NULL	DNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of 5-bromodeoxyuridine into DNA in newborn rat tissues .
	manualset3
99635	4	401093	13	NULL	NULL	0	NULL	newborn rat tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of 5-bromodeoxyuridine into DNA in newborn rat tissues .
	manualset3
99636	1	401094	13	NULL	NULL	0	NULL	Incorporation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of L - ( 1-ethyl - 14 C ) - and L - ( 35 S ) ethionine into mitochondrial proteins .
	manualset3
99637	2	401094	13	NULL	NULL	0	NULL	 L - ( 1-ethyl - 14 C ) ethionine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of L - ( 1-ethyl - 14 C ) - and L - ( 35 S ) ethionine into mitochondrial proteins .
	manualset3
99638	3	401094	13	NULL	NULL	0	NULL	L - ( 35 S ) ethionine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of L - ( 1-ethyl - 14 C ) - and L - ( 35 S ) ethionine into mitochondrial proteins .
	manualset3
99639	4	401094	13	NULL	NULL	0	NULL	mitochondrial proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of L - ( 1-ethyl - 14 C ) - and L - ( 35 S ) ethionine into mitochondrial proteins .
	manualset3
99640	1	401095	13	NULL	NULL	0	NULL	Incorporation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of SP-A into liposomes increased by 6.2-fold the delivery of liposomal SOD to cells .
	manualset3
99641	2	401095	13	NULL	NULL	0	NULL	SP-A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of SP-A into liposomes increased by 6.2-fold the delivery of liposomal SOD to cells .
	manualset3
99642	3	401095	13	NULL	NULL	0	NULL	liposomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of SP-A into liposomes increased by 6.2-fold the delivery of liposomal SOD to cells .
	manualset3
99643	4	401095	13	NULL	NULL	0	NULL	6.2-fold	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of SP-A into liposomes increased by 6.2-fold the delivery of liposomal SOD to cells .
	manualset3
99644	5	401095	13	NULL	NULL	0	NULL	liposomal SOD 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of SP-A into liposomes increased by 6.2-fold the delivery of liposomal SOD to cells .
	manualset3
99645	6	401095	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of SP-A into liposomes increased by 6.2-fold the delivery of liposomal SOD to cells .
	manualset3
99646	1	401096	13	NULL	NULL	0	NULL	Incorporation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of a single linker histone molecule into the nucleosome protects an additional 20 bp of linker DNA from micrococcal nuclease digestion .
	manualset3
99647	2	401096	13	NULL	NULL	0	NULL	single linker histone molecule	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of a single linker histone molecule into the nucleosome protects an additional 20 bp of linker DNA from micrococcal nuclease digestion .
	manualset3
99648	3	401096	13	NULL	NULL	0	NULL	nucleosome	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of a single linker histone molecule into the nucleosome protects an additional 20 bp of linker DNA from micrococcal nuclease digestion .
	manualset3
99649	4	401096	13	NULL	NULL	0	NULL	20 bp of linker DNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of a single linker histone molecule into the nucleosome protects an additional 20 bp of linker DNA from micrococcal nuclease digestion .
	manualset3
99650	5	401096	13	NULL	NULL	0	NULL	micrococcal nuclease digestion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of a single linker histone molecule into the nucleosome protects an additional 20 bp of linker DNA from micrococcal nuclease digestion .
	manualset3
99651	1	401097	13	NULL	NULL	0	NULL	Incorporation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of amino acids in vivo into brain total protein and into brain ribosomes was impaired , as was protein synthesis in vitro by microsomes isolated from the brain of poisoned rats .
	manualset3
99652	2	401097	13	NULL	NULL	0	NULL	amino acids 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of amino acids in vivo into brain total protein and into brain ribosomes was impaired , as was protein synthesis in vitro by microsomes isolated from the brain of poisoned rats .
	manualset3
99653	3	401097	13	NULL	NULL	NULL	NULL	brain total protein	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Incorporation of amino acids in vivo into brain total protein and into brain ribosomes was impaired , as was protein synthesis in vitro by microsomes isolated from the brain of poisoned rats .
	manualset3
99654	4	401097	13	NULL	NULL	0	NULL	brain ribosomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of amino acids in vivo into brain total protein and into brain ribosomes was impaired , as was protein synthesis in vitro by microsomes isolated from the brain of poisoned rats .
	manualset3
99655	5	401097	13	NULL	NULL	0	NULL	protein synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of amino acids in vivo into brain total protein and into brain ribosomes was impaired , as was protein synthesis in vitro by microsomes isolated from the brain of poisoned rats .
	manualset3
99656	6	401097	13	NULL	NULL	0	NULL	 microsomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of amino acids in vivo into brain total protein and into brain ribosomes was impaired , as was protein synthesis in vitro by microsomes isolated from the brain of poisoned rats .
	manualset3
99657	7	401097	13	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of amino acids in vivo into brain total protein and into brain ribosomes was impaired , as was protein synthesis in vitro by microsomes isolated from the brain of poisoned rats .
	manualset3
99658	8	401097	13	NULL	NULL	0	NULL	poisoned rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of amino acids in vivo into brain total protein and into brain ribosomes was impaired , as was protein synthesis in vitro by microsomes isolated from the brain of poisoned rats .
	manualset3
99659	1	401098	13	NULL	NULL	0	NULL	Incorporation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of such molecularly imprinted polymers ( MIPs ) in a platform suitable for electrochemical measurements , can offer high sensitivity together with device miniaturization and an electronic read-out .
	manualset3
99660	2	401098	13	NULL	NULL	0	NULL	molecularly imprinted polymers ( MIPs )	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of such molecularly imprinted polymers ( MIPs ) in a platform suitable for electrochemical measurements , can offer high sensitivity together with device miniaturization and an electronic read-out .
	manualset3
99661	3	401098	13	NULL	NULL	0	NULL	platform 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of such molecularly imprinted polymers ( MIPs ) in a platform suitable for electrochemical measurements , can offer high sensitivity together with device miniaturization and an electronic read-out .
	manualset3
99662	4	401098	13	NULL	NULL	0	NULL	electrochemical measurements 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of such molecularly imprinted polymers ( MIPs ) in a platform suitable for electrochemical measurements , can offer high sensitivity together with device miniaturization and an electronic read-out .
	manualset3
99665	5	401098	13	NULL	NULL	0	NULL	high sensitivity 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of such molecularly imprinted polymers ( MIPs ) in a platform suitable for electrochemical measurements , can offer high sensitivity together with device miniaturization and an electronic read-out .
	manualset3
99667	6	401098	13	NULL	NULL	0	NULL	device miniaturization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of such molecularly imprinted polymers ( MIPs ) in a platform suitable for electrochemical measurements , can offer high sensitivity together with device miniaturization and an electronic read-out .
	manualset3
99669	7	401098	13	NULL	NULL	0	NULL	electronic read-out	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of such molecularly imprinted polymers ( MIPs ) in a platform suitable for electrochemical measurements , can offer high sensitivity together with device miniaturization and an electronic read-out .
	manualset3
99671	1	401099	13	NULL	NULL	0	NULL	 L/M cones	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( 2 ) Heavily labeled L/M cones were wine goblet shaped with a small round cell body , a large nucleus at the outer ONL edge , and a thin axon with a prominent synaptic pedicle .
	manualset3
99672	2	401099	13	NULL	NULL	0	NULL	small round cell body 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	( 2 ) Heavily labeled L/M cones were wine goblet shaped with a small round cell body , a large nucleus at the outer ONL edge , and a thin axon with a prominent synaptic pedicle .
	manualset3
99673	3	401099	13	NULL	NULL	0	NULL	large nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	( 2 ) Heavily labeled L/M cones were wine goblet shaped with a small round cell body , a large nucleus at the outer ONL edge , and a thin axon with a prominent synaptic pedicle .
	manualset3
99674	4	401099	13	NULL	NULL	0	NULL	outer ONL edge	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	( 2 ) Heavily labeled L/M cones were wine goblet shaped with a small round cell body , a large nucleus at the outer ONL edge , and a thin axon with a prominent synaptic pedicle .
	manualset3
99675	5	401099	13	NULL	NULL	0	NULL	axon	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	( 2 ) Heavily labeled L/M cones were wine goblet shaped with a small round cell body , a large nucleus at the outer ONL edge , and a thin axon with a prominent synaptic pedicle .
	manualset3
99676	6	401099	13	NULL	NULL	0	NULL	synaptic pedicle	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	( 2 ) Heavily labeled L/M cones were wine goblet shaped with a small round cell body , a large nucleus at the outer ONL edge , and a thin axon with a prominent synaptic pedicle .
	manualset3
99677	1	401100	13	NULL	NULL	0	NULL	2	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	2 At concentrations greater than 2 x 10 ( -4 ) M , piperoxan produced a rise in perfusion pressure , a contraction of the splenic capsule , and a marked dose-dependent decrease in transmitter overflow .
	manualset3
99678	2	401100	13	NULL	NULL	0	NULL	concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 At concentrations greater than 2 x 10 ( -4 ) M , piperoxan produced a rise in perfusion pressure , a contraction of the splenic capsule , and a marked dose-dependent decrease in transmitter overflow .
	manualset3
99679	3	401100	13	NULL	NULL	0	NULL	2 x 10 ( -4 ) M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 At concentrations greater than 2 x 10 ( -4 ) M , piperoxan produced a rise in perfusion pressure , a contraction of the splenic capsule , and a marked dose-dependent decrease in transmitter overflow .
	manualset3
99680	4	401100	13	NULL	NULL	0	NULL	piperoxan	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	2 At concentrations greater than 2 x 10 ( -4 ) M , piperoxan produced a rise in perfusion pressure , a contraction of the splenic capsule , and a marked dose-dependent decrease in transmitter overflow .
	manualset3
99681	5	401100	13	NULL	NULL	0	NULL	rise in perfusion pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	2 At concentrations greater than 2 x 10 ( -4 ) M , piperoxan produced a rise in perfusion pressure , a contraction of the splenic capsule , and a marked dose-dependent decrease in transmitter overflow .
	manualset3
99682	6	401100	13	NULL	NULL	NULL	NULL	contraction of the splenic capsule	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	2 At concentrations greater than 2 x 10 ( -4 ) M , piperoxan produced a rise in perfusion pressure , a contraction of the splenic capsule , and a marked dose-dependent decrease in transmitter overflow .
	manualset3
99683	7	401100	13	NULL	NULL	0	NULL	decrease in transmitter overflow	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	2 At concentrations greater than 2 x 10 ( -4 ) M , piperoxan produced a rise in perfusion pressure , a contraction of the splenic capsule , and a marked dose-dependent decrease in transmitter overflow .
	manualset3
99684	1	401101	13	NULL	NULL	0	NULL	Increase in SCC 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increase in SCC by PRL accelerated as the stage advanced between stages XXII and XXV .
	manualset3
99685	2	401101	13	NULL	NULL	0	NULL	 PRL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Increase in SCC by PRL accelerated as the stage advanced between stages XXII and XXV .
	manualset3
99686	3	401101	13	NULL	NULL	0	NULL	 stage	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Increase in SCC by PRL accelerated as the stage advanced between stages XXII and XXV .
	manualset3
99687	4	401101	13	NULL	NULL	NULL	NULL	stage XXII	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Increase in SCC by PRL accelerated as the stage advanced between stages XXII and XXV .
	manualset3
99688	5	401101	13	NULL	NULL	0	NULL	 stage XXV	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Increase in SCC by PRL accelerated as the stage advanced between stages XXII and XXV .
	manualset3
99699	1	401102	13	NULL	NULL	0	NULL	 QTd	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased QTd , found in various cardiac diseases , reflects cardiac instability and is associated with increased risk for cardiac death .
	manualset3
99702	2	401102	13	NULL	NULL	NULL	NULL	cardiac diseases 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Increased QTd , found in various cardiac diseases , reflects cardiac instability and is associated with increased risk for cardiac death .
	manualset3
99705	3	401102	13	NULL	NULL	0	NULL	 cardiac instability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased QTd , found in various cardiac diseases , reflects cardiac instability and is associated with increased risk for cardiac death .
	manualset3
99706	4	401102	13	NULL	NULL	0	NULL	risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased QTd , found in various cardiac diseases , reflects cardiac instability and is associated with increased risk for cardiac death .
	manualset3
99707	5	401102	13	NULL	NULL	0	NULL	cardiac death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased QTd , found in various cardiac diseases , reflects cardiac instability and is associated with increased risk for cardiac death .
	manualset3
99710	1	401103	13	NULL	NULL	0	NULL	Diels-Alderase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased Diels-Alderase activity through backbone remodeling guided by Foldit players .
	manualset3
99714	2	401103	13	NULL	NULL	0	NULL	backbone remodeling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased Diels-Alderase activity through backbone remodeling guided by Foldit players .
	manualset3
99716	3	401103	13	NULL	NULL	0	NULL	Foldit players	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased Diels-Alderase activity through backbone remodeling guided by Foldit players .
	manualset3
99720	1	401104	13	NULL	NULL	0	NULL	MT synthesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased MT synthesis in the liver may contribute to copper detoxification ; the hypothesis of copper entrapment in enterocytes can not be confirmed .
	manualset3
99722	2	401104	13	NULL	NULL	0	NULL	 liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased MT synthesis in the liver may contribute to copper detoxification ; the hypothesis of copper entrapment in enterocytes can not be confirmed .
	manualset3
99723	3	401104	13	NULL	NULL	NULL	NULL	copper detoxification	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Increased MT synthesis in the liver may contribute to copper detoxification ; the hypothesis of copper entrapment in enterocytes can not be confirmed .
	manualset3
99724	4	401104	13	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased MT synthesis in the liver may contribute to copper detoxification ; the hypothesis of copper entrapment in enterocytes can not be confirmed .
	manualset3
99725	5	401104	13	NULL	NULL	0	NULL	copper entrapment	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased MT synthesis in the liver may contribute to copper detoxification ; the hypothesis of copper entrapment in enterocytes can not be confirmed .
	manualset3
99726	6	401104	13	NULL	NULL	0	NULL	 enterocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased MT synthesis in the liver may contribute to copper detoxification ; the hypothesis of copper entrapment in enterocytes can not be confirmed .
	manualset3
99727	1	401105	13	NULL	NULL	0	NULL	Na + , K + - ATPase activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased Na + , K + - ATPase activity observed after chronic ethanol consumption has been examined to determine whether the increase is due to changes in the kinetic properties of the enzyme or increases in the amount of enzyme in the membranes examined .
	manualset3
99728	2	401105	13	NULL	NULL	0	NULL	chronic ethanol consumption	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased Na + , K + - ATPase activity observed after chronic ethanol consumption has been examined to determine whether the increase is due to changes in the kinetic properties of the enzyme or increases in the amount of enzyme in the membranes examined .
	manualset3
99729	3	401105	13	NULL	NULL	0	NULL	changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased Na + , K + - ATPase activity observed after chronic ethanol consumption has been examined to determine whether the increase is due to changes in the kinetic properties of the enzyme or increases in the amount of enzyme in the membranes examined .
	manualset3
99730	4	401105	13	NULL	NULL	0	NULL	kinetic properties of the enzyme	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased Na + , K + - ATPase activity observed after chronic ethanol consumption has been examined to determine whether the increase is due to changes in the kinetic properties of the enzyme or increases in the amount of enzyme in the membranes examined .
	manualset3
99731	5	401105	13	NULL	NULL	0	NULL	amount of enzyme	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased Na + , K + - ATPase activity observed after chronic ethanol consumption has been examined to determine whether the increase is due to changes in the kinetic properties of the enzyme or increases in the amount of enzyme in the membranes examined .
	manualset3
99732	6	401105	13	NULL	NULL	0	NULL	membranes 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased Na + , K + - ATPase activity observed after chronic ethanol consumption has been examined to determine whether the increase is due to changes in the kinetic properties of the enzyme or increases in the amount of enzyme in the membranes examined .
	manualset3
99734	1	401106	13	NULL	NULL	0	NULL	 activity of citrate synthase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased activity of citrate synthase in human skeletal muscle after a single bout of prolonged exercise .
	manualset3
99735	2	401106	13	NULL	NULL	0	NULL	human skeletal muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased activity of citrate synthase in human skeletal muscle after a single bout of prolonged exercise .
	manualset3
99736	3	401106	13	NULL	NULL	0	NULL	single bout	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased activity of citrate synthase in human skeletal muscle after a single bout of prolonged exercise .
	manualset3
99737	4	401106	13	NULL	NULL	0	NULL	exercise 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased activity of citrate synthase in human skeletal muscle after a single bout of prolonged exercise .
	manualset3
99741	1	401107	13	NULL	NULL	0	NULL	antitumor action 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased antitumor action of nitrogen mutard caused by induced hypothyroidism .
	manualset3
99742	2	401107	13	NULL	NULL	0	NULL	nitrogen mutard	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased antitumor action of nitrogen mutard caused by induced hypothyroidism .
	manualset3
99744	3	401107	13	NULL	NULL	0	NULL	hypothyroidism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased antitumor action of nitrogen mutard caused by induced hypothyroidism .
	manualset3
99746	1	401108	13	NULL	NULL	0	NULL	Digitoxin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	2 Digitoxin produced the greatest inotropic responses in this series , while the sequence of cleavage products produced progressively smaller responses .
	manualset3
99747	2	401108	13	NULL	NULL	NULL	NULL	inotropic responses	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	2 Digitoxin produced the greatest inotropic responses in this series , while the sequence of cleavage products produced progressively smaller responses .
	manualset3
99748	3	401108	13	NULL	NULL	0	NULL	series	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	2 Digitoxin produced the greatest inotropic responses in this series , while the sequence of cleavage products produced progressively smaller responses .
	manualset3
99749	4	401108	13	NULL	NULL	NULL	NULL	sequence of cleavage products	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	2 Digitoxin produced the greatest inotropic responses in this series , while the sequence of cleavage products produced progressively smaller responses .
	manualset3
99750	5	401108	13	NULL	NULL	NULL	NULL	smaller responses	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	2 Digitoxin produced the greatest inotropic responses in this series , while the sequence of cleavage products produced progressively smaller responses .
	manualset3
99751	1	401109	13	NULL	NULL	0	NULL	levels of endogenous ouabain ( EO ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased circulating levels of endogenous ouabain ( EO ) have been observed in some heart failure patients , but their long term clinical significance is unknown .
	manualset3
99752	2	401109	13	NULL	NULL	0	NULL	heart failure patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased circulating levels of endogenous ouabain ( EO ) have been observed in some heart failure patients , but their long term clinical significance is unknown .
	manualset3
99753	3	401109	13	NULL	NULL	0	NULL	long term	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased circulating levels of endogenous ouabain ( EO ) have been observed in some heart failure patients , but their long term clinical significance is unknown .
	manualset3
99754	4	401109	13	NULL	NULL	0	NULL	clinical significance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased circulating levels of endogenous ouabain ( EO ) have been observed in some heart failure patients , but their long term clinical significance is unknown .
	manualset3
99755	1	401110	13	NULL	NULL	0	NULL	consumption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased consumption of polyunsaturated fat leads to pronounced reduction in plasma triglyceride concentrations .
	manualset3
99756	2	401110	13	NULL	NULL	0	NULL	polyunsaturated fat	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased consumption of polyunsaturated fat leads to pronounced reduction in plasma triglyceride concentrations .
	manualset3
99757	3	401110	13	NULL	NULL	0	NULL	leads	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased consumption of polyunsaturated fat leads to pronounced reduction in plasma triglyceride concentrations .
	manualset3
99758	4	401110	13	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased consumption of polyunsaturated fat leads to pronounced reduction in plasma triglyceride concentrations .
	manualset3
99759	5	401110	13	NULL	NULL	0	NULL	plasma triglyceride concentrations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased consumption of polyunsaturated fat leads to pronounced reduction in plasma triglyceride concentrations .
	manualset3
99779	1	401111	13	NULL	NULL	0	NULL	donor 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased donor age was a significant risk factor for death and graft loss among all age groups after deceased donor kidney transplantation but not among living-donor kidney recipients .
	manualset3
99780	2	401111	13	NULL	NULL	0	NULL	age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased donor age was a significant risk factor for death and graft loss among all age groups after deceased donor kidney transplantation but not among living-donor kidney recipients .
	manualset3
99783	3	401111	13	NULL	NULL	0	NULL	 risk factor 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased donor age was a significant risk factor for death and graft loss among all age groups after deceased donor kidney transplantation but not among living-donor kidney recipients .
	manualset3
99784	4	401111	13	NULL	NULL	0	NULL	 death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased donor age was a significant risk factor for death and graft loss among all age groups after deceased donor kidney transplantation but not among living-donor kidney recipients .
	manualset3
99785	5	401111	13	NULL	NULL	0	NULL	 graft loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased donor age was a significant risk factor for death and graft loss among all age groups after deceased donor kidney transplantation but not among living-donor kidney recipients .
	manualset3
99786	6	401111	13	NULL	NULL	0	NULL	all age groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased donor age was a significant risk factor for death and graft loss among all age groups after deceased donor kidney transplantation but not among living-donor kidney recipients .
	manualset3
99787	7	401111	13	NULL	NULL	0	NULL	donor	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased donor age was a significant risk factor for death and graft loss among all age groups after deceased donor kidney transplantation but not among living-donor kidney recipients .
	manualset3
99788	8	401111	13	NULL	NULL	0	NULL	kidney transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased donor age was a significant risk factor for death and graft loss among all age groups after deceased donor kidney transplantation but not among living-donor kidney recipients .
	manualset3
99789	9	401111	13	NULL	NULL	0	NULL	living-donor kidney recipients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased donor age was a significant risk factor for death and graft loss among all age groups after deceased donor kidney transplantation but not among living-donor kidney recipients .
	manualset3
99790	1	401112	13	NULL	NULL	0	NULL	endogenous catalase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased endogenous catalase preserves CK during RP , resulting in normal function and bioenergetics .
	manualset3
99791	2	401112	13	NULL	NULL	0	NULL	 preserves	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased endogenous catalase preserves CK during RP , resulting in normal function and bioenergetics .
	manualset3
99792	3	401112	13	NULL	NULL	0	NULL	CK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased endogenous catalase preserves CK during RP , resulting in normal function and bioenergetics .
	manualset3
99793	4	401112	13	NULL	NULL	0	NULL	RP	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased endogenous catalase preserves CK during RP , resulting in normal function and bioenergetics .
	manualset3
99794	5	401112	13	NULL	NULL	0	NULL	normal function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased endogenous catalase preserves CK during RP , resulting in normal function and bioenergetics .
	manualset3
99795	6	401112	13	NULL	NULL	0	NULL	bioenergetics	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased endogenous catalase preserves CK during RP , resulting in normal function and bioenergetics .
	manualset3
99796	1	401113	13	NULL	NULL	0	NULL	 excretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased excretion of urinary porphyrins by white rats given intragastrically the chemical carcinogens diethylnitrosamine , monocrotaline , T-2 toxin and ethylmethanesulphonate ( proceedings ) .
	manualset3
99797	2	401113	13	NULL	NULL	0	NULL	 urinary porphyrins 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased excretion of urinary porphyrins by white rats given intragastrically the chemical carcinogens diethylnitrosamine , monocrotaline , T-2 toxin and ethylmethanesulphonate ( proceedings ) .
	manualset3
99798	3	401113	13	NULL	NULL	0	NULL	white rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased excretion of urinary porphyrins by white rats given intragastrically the chemical carcinogens diethylnitrosamine , monocrotaline , T-2 toxin and ethylmethanesulphonate ( proceedings ) .
	manualset3
99799	4	401113	13	NULL	NULL	0	NULL	chemical carcinogens	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased excretion of urinary porphyrins by white rats given intragastrically the chemical carcinogens diethylnitrosamine , monocrotaline , T-2 toxin and ethylmethanesulphonate ( proceedings ) .
	manualset3
99800	5	401113	13	NULL	NULL	0	NULL	diethylnitrosamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased excretion of urinary porphyrins by white rats given intragastrically the chemical carcinogens diethylnitrosamine , monocrotaline , T-2 toxin and ethylmethanesulphonate ( proceedings ) .
	manualset3
99801	6	401113	13	NULL	NULL	0	NULL	monocrotaline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased excretion of urinary porphyrins by white rats given intragastrically the chemical carcinogens diethylnitrosamine , monocrotaline , T-2 toxin and ethylmethanesulphonate ( proceedings ) .
	manualset3
99802	7	401113	13	NULL	NULL	0	NULL	T-2 toxin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased excretion of urinary porphyrins by white rats given intragastrically the chemical carcinogens diethylnitrosamine , monocrotaline , T-2 toxin and ethylmethanesulphonate ( proceedings ) .
	manualset3
99803	8	401113	13	NULL	NULL	0	NULL	 ethylmethanesulphonate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased excretion of urinary porphyrins by white rats given intragastrically the chemical carcinogens diethylnitrosamine , monocrotaline , T-2 toxin and ethylmethanesulphonate ( proceedings ) .
	manualset3
99804	9	401113	13	NULL	NULL	0	NULL	proceedings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased excretion of urinary porphyrins by white rats given intragastrically the chemical carcinogens diethylnitrosamine , monocrotaline , T-2 toxin and ethylmethanesulphonate ( proceedings ) .
	manualset3
99805	1	401114	13	NULL	NULL	0	NULL	expression of CC chemokine ligand 18	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased expression of CC chemokine ligand 18 in patients with chronic rhinosinusitis with nasal polyps .
	manualset3
99806	2	401114	13	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased expression of CC chemokine ligand 18 in patients with chronic rhinosinusitis with nasal polyps .
	manualset3
99807	3	401114	13	NULL	NULL	0	NULL	chronic rhinosinusitis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased expression of CC chemokine ligand 18 in patients with chronic rhinosinusitis with nasal polyps .
	manualset3
99808	4	401114	13	NULL	NULL	0	NULL	nasal polyps	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased expression of CC chemokine ligand 18 in patients with chronic rhinosinusitis with nasal polyps .
	manualset3
99809	1	401115	13	NULL	NULL	0	NULL	fluorine-18 fluorodeoxyglucose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased fluorine-18 fluorodeoxyglucose uptake in the right atrial wall in a patient with atrial fibrillation .
	manualset3
99818	2	401115	13	NULL	NULL	0	NULL	uptake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased fluorine-18 fluorodeoxyglucose uptake in the right atrial wall in a patient with atrial fibrillation .
	manualset3
99819	3	401115	13	NULL	NULL	0	NULL	right atrial wall 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased fluorine-18 fluorodeoxyglucose uptake in the right atrial wall in a patient with atrial fibrillation .
	manualset3
99820	4	401115	13	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased fluorine-18 fluorodeoxyglucose uptake in the right atrial wall in a patient with atrial fibrillation .
	manualset3
99825	5	401115	13	NULL	NULL	0	NULL	atrial fibrillation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased fluorine-18 fluorodeoxyglucose uptake in the right atrial wall in a patient with atrial fibrillation .
	manualset3
99832	1	401116	13	NULL	NULL	0	NULL	gastrointestinal permeability 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased gastrointestinal permeability in patients with Plasmodium falciparum malaria .
	manualset3
99833	2	401116	13	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased gastrointestinal permeability in patients with Plasmodium falciparum malaria .
	manualset3
99834	3	401116	13	NULL	NULL	0	NULL	Plasmodium falciparum malaria	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased gastrointestinal permeability in patients with Plasmodium falciparum malaria .
	manualset3
99835	1	401117	13	NULL	NULL	0	NULL	2 insurers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	2 insurers drop from HIAA to tout their own reform ideas .
	manualset3
99836	2	401117	13	NULL	NULL	0	NULL	HIAA	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	2 insurers drop from HIAA to tout their own reform ideas .
	manualset3
99837	3	401117	13	NULL	NULL	0	NULL	reform ideas	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	2 insurers drop from HIAA to tout their own reform ideas .
	manualset3
99838	1	401118	13	NULL	NULL	NULL	NULL	glutamatergic input 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Increased glutamatergic input in the paraventricular nucleus ( PVN ) is important for high sympathetic outflow in hypertension , but the associated molecular mechanisms remain unclear .
	manualset3
99839	2	401118	13	NULL	NULL	0	NULL	paraventricular nucleus ( PVN )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased glutamatergic input in the paraventricular nucleus ( PVN ) is important for high sympathetic outflow in hypertension , but the associated molecular mechanisms remain unclear .
	manualset3
99846	3	401118	13	NULL	NULL	0	NULL	sympathetic outflow 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased glutamatergic input in the paraventricular nucleus ( PVN ) is important for high sympathetic outflow in hypertension , but the associated molecular mechanisms remain unclear .
	manualset3
99847	4	401118	13	NULL	NULL	0	NULL	 hypertension 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased glutamatergic input in the paraventricular nucleus ( PVN ) is important for high sympathetic outflow in hypertension , but the associated molecular mechanisms remain unclear .
	manualset3
99848	5	401118	13	NULL	NULL	0	NULL	molecular mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased glutamatergic input in the paraventricular nucleus ( PVN ) is important for high sympathetic outflow in hypertension , but the associated molecular mechanisms remain unclear .
	manualset3
99849	1	401119	13	NULL	NULL	0	NULL	levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels in vivo of mRNAs for IL-8 and macrophage inflammatory protein-1 alpha ( MIP-1 alpha ) , but not of RANTES mRNA in peripheral blood mononuclear cells of patients with atopic dermatitis ( AD ) .
	manualset3
99850	2	401119	13	NULL	NULL	0	NULL	mRNAs for IL-8	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels in vivo of mRNAs for IL-8 and macrophage inflammatory protein-1 alpha ( MIP-1 alpha ) , but not of RANTES mRNA in peripheral blood mononuclear cells of patients with atopic dermatitis ( AD ) .
	manualset3
99851	3	401119	13	NULL	NULL	0	NULL	mRNAs macrophage inflammatory protein-1 alpha ( MIP-1 alpha )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels in vivo of mRNAs for IL-8 and macrophage inflammatory protein-1 alpha ( MIP-1 alpha ) , but not of RANTES mRNA in peripheral blood mononuclear cells of patients with atopic dermatitis ( AD ) .
	manualset3
99852	4	401119	13	NULL	NULL	0	NULL	RANTES mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels in vivo of mRNAs for IL-8 and macrophage inflammatory protein-1 alpha ( MIP-1 alpha ) , but not of RANTES mRNA in peripheral blood mononuclear cells of patients with atopic dermatitis ( AD ) .
	manualset3
99853	5	401119	13	NULL	NULL	0	NULL	peripheral blood mononuclear cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels in vivo of mRNAs for IL-8 and macrophage inflammatory protein-1 alpha ( MIP-1 alpha ) , but not of RANTES mRNA in peripheral blood mononuclear cells of patients with atopic dermatitis ( AD ) .
	manualset3
99854	6	401119	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels in vivo of mRNAs for IL-8 and macrophage inflammatory protein-1 alpha ( MIP-1 alpha ) , but not of RANTES mRNA in peripheral blood mononuclear cells of patients with atopic dermatitis ( AD ) .
	manualset3
99855	7	401119	13	NULL	NULL	0	NULL	atopic dermatitis ( AD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels in vivo of mRNAs for IL-8 and macrophage inflammatory protein-1 alpha ( MIP-1 alpha ) , but not of RANTES mRNA in peripheral blood mononuclear cells of patients with atopic dermatitis ( AD ) .
	manualset3
99856	1	401120	13	NULL	NULL	0	NULL	levels of ROS	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of ROS and cell death induced by H2AX overexpression alone or DNA damage leading to H2AX accumulation are reduced by treating cells with the antioxidant N-Acetyl-L-Cysteine ( NAC ) , the NADP ( H ) oxidase ( Nox ) inhibitor DPI , expression of Rac1N17 , and knockdown of Nox1 , but not Nox4 , indicating that induction of ROS by H2AX is mediated through Nox1 and Rac1 GTPase .
	manualset3
99857	2	401120	13	NULL	NULL	0	NULL	cell death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of ROS and cell death induced by H2AX overexpression alone or DNA damage leading to H2AX accumulation are reduced by treating cells with the antioxidant N-Acetyl-L-Cysteine ( NAC ) , the NADP ( H ) oxidase ( Nox ) inhibitor DPI , expression of Rac1N17 , and knockdown of Nox1 , but not Nox4 , indicating that induction of ROS by H2AX is mediated through Nox1 and Rac1 GTPase .
	manualset3
99858	3	401120	13	NULL	NULL	0	NULL	H2AX overexpression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of ROS and cell death induced by H2AX overexpression alone or DNA damage leading to H2AX accumulation are reduced by treating cells with the antioxidant N-Acetyl-L-Cysteine ( NAC ) , the NADP ( H ) oxidase ( Nox ) inhibitor DPI , expression of Rac1N17 , and knockdown of Nox1 , but not Nox4 , indicating that induction of ROS by H2AX is mediated through Nox1 and Rac1 GTPase .
	manualset3
99859	4	401120	13	NULL	NULL	0	NULL	DNA damage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of ROS and cell death induced by H2AX overexpression alone or DNA damage leading to H2AX accumulation are reduced by treating cells with the antioxidant N-Acetyl-L-Cysteine ( NAC ) , the NADP ( H ) oxidase ( Nox ) inhibitor DPI , expression of Rac1N17 , and knockdown of Nox1 , but not Nox4 , indicating that induction of ROS by H2AX is mediated through Nox1 and Rac1 GTPase .
	manualset3
99860	5	401120	13	NULL	NULL	0	NULL	H2AX accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of ROS and cell death induced by H2AX overexpression alone or DNA damage leading to H2AX accumulation are reduced by treating cells with the antioxidant N-Acetyl-L-Cysteine ( NAC ) , the NADP ( H ) oxidase ( Nox ) inhibitor DPI , expression of Rac1N17 , and knockdown of Nox1 , but not Nox4 , indicating that induction of ROS by H2AX is mediated through Nox1 and Rac1 GTPase .
	manualset3
99861	6	401120	13	NULL	NULL	0	NULL	 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of ROS and cell death induced by H2AX overexpression alone or DNA damage leading to H2AX accumulation are reduced by treating cells with the antioxidant N-Acetyl-L-Cysteine ( NAC ) , the NADP ( H ) oxidase ( Nox ) inhibitor DPI , expression of Rac1N17 , and knockdown of Nox1 , but not Nox4 , indicating that induction of ROS by H2AX is mediated through Nox1 and Rac1 GTPase .
	manualset3
99862	7	401120	13	NULL	NULL	0	NULL	antioxidant N-Acetyl-L-Cysteine ( NAC )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of ROS and cell death induced by H2AX overexpression alone or DNA damage leading to H2AX accumulation are reduced by treating cells with the antioxidant N-Acetyl-L-Cysteine ( NAC ) , the NADP ( H ) oxidase ( Nox ) inhibitor DPI , expression of Rac1N17 , and knockdown of Nox1 , but not Nox4 , indicating that induction of ROS by H2AX is mediated through Nox1 and Rac1 GTPase .
	manualset3
99863	8	401120	13	NULL	NULL	0	NULL	NADP ( H ) oxidase ( Nox ) inhibitor DPI 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of ROS and cell death induced by H2AX overexpression alone or DNA damage leading to H2AX accumulation are reduced by treating cells with the antioxidant N-Acetyl-L-Cysteine ( NAC ) , the NADP ( H ) oxidase ( Nox ) inhibitor DPI , expression of Rac1N17 , and knockdown of Nox1 , but not Nox4 , indicating that induction of ROS by H2AX is mediated through Nox1 and Rac1 GTPase .
	manualset3
99864	9	401120	13	NULL	NULL	0	NULL	expression of Rac1N17	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of ROS and cell death induced by H2AX overexpression alone or DNA damage leading to H2AX accumulation are reduced by treating cells with the antioxidant N-Acetyl-L-Cysteine ( NAC ) , the NADP ( H ) oxidase ( Nox ) inhibitor DPI , expression of Rac1N17 , and knockdown of Nox1 , but not Nox4 , indicating that induction of ROS by H2AX is mediated through Nox1 and Rac1 GTPase .
	manualset3
99865	10	401120	13	NULL	NULL	0	NULL	knockdown of Nox1	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of ROS and cell death induced by H2AX overexpression alone or DNA damage leading to H2AX accumulation are reduced by treating cells with the antioxidant N-Acetyl-L-Cysteine ( NAC ) , the NADP ( H ) oxidase ( Nox ) inhibitor DPI , expression of Rac1N17 , and knockdown of Nox1 , but not Nox4 , indicating that induction of ROS by H2AX is mediated through Nox1 and Rac1 GTPase .
	manualset3
99866	11	401120	13	NULL	NULL	0	NULL	 Nox4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of ROS and cell death induced by H2AX overexpression alone or DNA damage leading to H2AX accumulation are reduced by treating cells with the antioxidant N-Acetyl-L-Cysteine ( NAC ) , the NADP ( H ) oxidase ( Nox ) inhibitor DPI , expression of Rac1N17 , and knockdown of Nox1 , but not Nox4 , indicating that induction of ROS by H2AX is mediated through Nox1 and Rac1 GTPase .
	manualset3
99867	12	401120	13	NULL	NULL	0	NULL	induction of ROS	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of ROS and cell death induced by H2AX overexpression alone or DNA damage leading to H2AX accumulation are reduced by treating cells with the antioxidant N-Acetyl-L-Cysteine ( NAC ) , the NADP ( H ) oxidase ( Nox ) inhibitor DPI , expression of Rac1N17 , and knockdown of Nox1 , but not Nox4 , indicating that induction of ROS by H2AX is mediated through Nox1 and Rac1 GTPase .
	manualset3
99868	13	401120	13	NULL	NULL	0	NULL	H2AX	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of ROS and cell death induced by H2AX overexpression alone or DNA damage leading to H2AX accumulation are reduced by treating cells with the antioxidant N-Acetyl-L-Cysteine ( NAC ) , the NADP ( H ) oxidase ( Nox ) inhibitor DPI , expression of Rac1N17 , and knockdown of Nox1 , but not Nox4 , indicating that induction of ROS by H2AX is mediated through Nox1 and Rac1 GTPase .
	manualset3
99869	14	401120	13	NULL	NULL	0	NULL	Nox1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of ROS and cell death induced by H2AX overexpression alone or DNA damage leading to H2AX accumulation are reduced by treating cells with the antioxidant N-Acetyl-L-Cysteine ( NAC ) , the NADP ( H ) oxidase ( Nox ) inhibitor DPI , expression of Rac1N17 , and knockdown of Nox1 , but not Nox4 , indicating that induction of ROS by H2AX is mediated through Nox1 and Rac1 GTPase .
	manualset3
99870	15	401120	13	NULL	NULL	0	NULL	Rac1 GTPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of ROS and cell death induced by H2AX overexpression alone or DNA damage leading to H2AX accumulation are reduced by treating cells with the antioxidant N-Acetyl-L-Cysteine ( NAC ) , the NADP ( H ) oxidase ( Nox ) inhibitor DPI , expression of Rac1N17 , and knockdown of Nox1 , but not Nox4 , indicating that induction of ROS by H2AX is mediated through Nox1 and Rac1 GTPase .
	manualset3
99871	1	401121	13	NULL	NULL	0	NULL	levels of hepatic iron	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of hepatic iron may impair the response of patients with chronic hepatitis C to treatment with interferon-alfa , but combination therapy with ribavirin has demonstrated efficacy in the treatment of hepatitis C. When used alone or with interferon-alfa , ribavirin may cause a dose-dependent reversible hemolytic anemia .
	manualset3
99872	2	401121	13	NULL	NULL	0	NULL	response 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of hepatic iron may impair the response of patients with chronic hepatitis C to treatment with interferon-alfa , but combination therapy with ribavirin has demonstrated efficacy in the treatment of hepatitis C. When used alone or with interferon-alfa , ribavirin may cause a dose-dependent reversible hemolytic anemia .
	manualset3
99873	3	401121	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of hepatic iron may impair the response of patients with chronic hepatitis C to treatment with interferon-alfa , but combination therapy with ribavirin has demonstrated efficacy in the treatment of hepatitis C. When used alone or with interferon-alfa , ribavirin may cause a dose-dependent reversible hemolytic anemia .
	manualset3
99874	4	401121	13	NULL	NULL	0	NULL	chronic hepatitis C	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of hepatic iron may impair the response of patients with chronic hepatitis C to treatment with interferon-alfa , but combination therapy with ribavirin has demonstrated efficacy in the treatment of hepatitis C. When used alone or with interferon-alfa , ribavirin may cause a dose-dependent reversible hemolytic anemia .
	manualset3
99875	5	401121	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of hepatic iron may impair the response of patients with chronic hepatitis C to treatment with interferon-alfa , but combination therapy with ribavirin has demonstrated efficacy in the treatment of hepatitis C. When used alone or with interferon-alfa , ribavirin may cause a dose-dependent reversible hemolytic anemia .
	manualset3
99876	6	401121	13	NULL	NULL	0	NULL	 interferon-alfa	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of hepatic iron may impair the response of patients with chronic hepatitis C to treatment with interferon-alfa , but combination therapy with ribavirin has demonstrated efficacy in the treatment of hepatitis C. When used alone or with interferon-alfa , ribavirin may cause a dose-dependent reversible hemolytic anemia .
	manualset3
99877	7	401121	13	NULL	NULL	0	NULL	combination therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of hepatic iron may impair the response of patients with chronic hepatitis C to treatment with interferon-alfa , but combination therapy with ribavirin has demonstrated efficacy in the treatment of hepatitis C. When used alone or with interferon-alfa , ribavirin may cause a dose-dependent reversible hemolytic anemia .
	manualset3
99878	8	401121	13	NULL	NULL	0	NULL	ribavirin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of hepatic iron may impair the response of patients with chronic hepatitis C to treatment with interferon-alfa , but combination therapy with ribavirin has demonstrated efficacy in the treatment of hepatitis C. When used alone or with interferon-alfa , ribavirin may cause a dose-dependent reversible hemolytic anemia .
	manualset3
99879	9	401121	13	NULL	NULL	0	NULL	 efficacy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of hepatic iron may impair the response of patients with chronic hepatitis C to treatment with interferon-alfa , but combination therapy with ribavirin has demonstrated efficacy in the treatment of hepatitis C. When used alone or with interferon-alfa , ribavirin may cause a dose-dependent reversible hemolytic anemia .
	manualset3
99880	10	401121	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of hepatic iron may impair the response of patients with chronic hepatitis C to treatment with interferon-alfa , but combination therapy with ribavirin has demonstrated efficacy in the treatment of hepatitis C. When used alone or with interferon-alfa , ribavirin may cause a dose-dependent reversible hemolytic anemia .
	manualset3
99881	11	401121	13	NULL	NULL	0	NULL	hepatitis C	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of hepatic iron may impair the response of patients with chronic hepatitis C to treatment with interferon-alfa , but combination therapy with ribavirin has demonstrated efficacy in the treatment of hepatitis C. When used alone or with interferon-alfa , ribavirin may cause a dose-dependent reversible hemolytic anemia .
	manualset3
99882	12	401121	13	NULL	NULL	0	NULL	interferon-alfa	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of hepatic iron may impair the response of patients with chronic hepatitis C to treatment with interferon-alfa , but combination therapy with ribavirin has demonstrated efficacy in the treatment of hepatitis C. When used alone or with interferon-alfa , ribavirin may cause a dose-dependent reversible hemolytic anemia .
	manualset3
99883	13	401121	13	NULL	NULL	0	NULL	ribavirin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of hepatic iron may impair the response of patients with chronic hepatitis C to treatment with interferon-alfa , but combination therapy with ribavirin has demonstrated efficacy in the treatment of hepatitis C. When used alone or with interferon-alfa , ribavirin may cause a dose-dependent reversible hemolytic anemia .
	manualset3
99884	14	401121	13	NULL	NULL	0	NULL	hemolytic anemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased levels of hepatic iron may impair the response of patients with chronic hepatitis C to treatment with interferon-alfa , but combination therapy with ribavirin has demonstrated efficacy in the treatment of hepatitis C. When used alone or with interferon-alfa , ribavirin may cause a dose-dependent reversible hemolytic anemia .
	manualset3
99885	1	401122	13	NULL	NULL	0	NULL	metastasis formation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased metastasis formation seemed to result from the selection of cells with increased resistance to nonspecific host effector cells .
	manualset3
99886	2	401122	13	NULL	NULL	0	NULL	selection of cells	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased metastasis formation seemed to result from the selection of cells with increased resistance to nonspecific host effector cells .
	manualset3
99887	3	401122	13	NULL	NULL	0	NULL	resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased metastasis formation seemed to result from the selection of cells with increased resistance to nonspecific host effector cells .
	manualset3
99888	4	401122	13	NULL	NULL	0	NULL	nonspecific host effector cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased metastasis formation seemed to result from the selection of cells with increased resistance to nonspecific host effector cells .
	manualset3
99889	1	401123	13	NULL	NULL	0	NULL	number	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased number of secondary fixed wing ( FW ) operations and more use of rotor wing ( RW ) transports .
	manualset3
99890	2	401123	13	NULL	NULL	0	NULL	secondary fixed wing ( FW ) operations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased number of secondary fixed wing ( FW ) operations and more use of rotor wing ( RW ) transports .
	manualset3
99891	3	401123	13	NULL	NULL	0	NULL	rotor wing ( RW ) transports	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased number of secondary fixed wing ( FW ) operations and more use of rotor wing ( RW ) transports .
	manualset3
99892	1	401124	13	NULL	NULL	0	NULL	numbers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased numbers of eosinophils frequently demarcated the mast cell infiltrates from the surrounding tissue .
	manualset3
99893	2	401124	13	NULL	NULL	0	NULL	eosinophils	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased numbers of eosinophils frequently demarcated the mast cell infiltrates from the surrounding tissue .
	manualset3
99894	3	401124	13	NULL	NULL	0	NULL	mast cell infiltrates	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased numbers of eosinophils frequently demarcated the mast cell infiltrates from the surrounding tissue .
	manualset3
99895	4	401124	13	NULL	NULL	0	NULL	tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased numbers of eosinophils frequently demarcated the mast cell infiltrates from the surrounding tissue .
	manualset3
99896	1	401125	13	NULL	NULL	0	NULL	p53	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased p53 mutation frequency during tumor progression -- results from a breast cancer cohort .
	manualset3
99897	2	401125	13	NULL	NULL	0	NULL	mutation frequency 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased p53 mutation frequency during tumor progression -- results from a breast cancer cohort .
	manualset3
99898	3	401125	13	NULL	NULL	0	NULL	tumor progression 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased p53 mutation frequency during tumor progression -- results from a breast cancer cohort .
	manualset3
99899	4	401125	13	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased p53 mutation frequency during tumor progression -- results from a breast cancer cohort .
	manualset3
99900	5	401125	13	NULL	NULL	0	NULL	breast cancer cohort 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased p53 mutation frequency during tumor progression -- results from a breast cancer cohort .
	manualset3
99901	1	401126	13	NULL	NULL	0	NULL	 plasma levels of prostaglandin D2	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased plasma levels of prostaglandin D2 and blood histamine after heat challenge indicate a role for mast cell degranulation in the pathophysiology of the syndrome .
	manualset3
99902	2	401126	13	NULL	NULL	0	NULL	 blood histamine	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased plasma levels of prostaglandin D2 and blood histamine after heat challenge indicate a role for mast cell degranulation in the pathophysiology of the syndrome .
	manualset3
99903	3	401126	13	NULL	NULL	0	NULL	heat challenge	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased plasma levels of prostaglandin D2 and blood histamine after heat challenge indicate a role for mast cell degranulation in the pathophysiology of the syndrome .
	manualset3
99904	4	401126	13	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased plasma levels of prostaglandin D2 and blood histamine after heat challenge indicate a role for mast cell degranulation in the pathophysiology of the syndrome .
	manualset3
99905	5	401126	13	NULL	NULL	0	NULL	mast cell degranulation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased plasma levels of prostaglandin D2 and blood histamine after heat challenge indicate a role for mast cell degranulation in the pathophysiology of the syndrome .
	manualset3
99906	6	401126	13	NULL	NULL	0	NULL	pathophysiology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased plasma levels of prostaglandin D2 and blood histamine after heat challenge indicate a role for mast cell degranulation in the pathophysiology of the syndrome .
	manualset3
99907	7	401126	13	NULL	NULL	0	NULL	syndrome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased plasma levels of prostaglandin D2 and blood histamine after heat challenge indicate a role for mast cell degranulation in the pathophysiology of the syndrome .
	manualset3
99908	1	401127	13	NULL	NULL	0	NULL	rates of detachment 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased rates of detachment depend on dynein activity , supporting previous evidence that She1 inhibits dynein .
	manualset3
99909	2	401127	13	NULL	NULL	0	NULL	dynein activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased rates of detachment depend on dynein activity , supporting previous evidence that She1 inhibits dynein .
	manualset3
99910	3	401127	13	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased rates of detachment depend on dynein activity , supporting previous evidence that She1 inhibits dynein .
	manualset3
99911	4	401127	13	NULL	NULL	0	NULL	She1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased rates of detachment depend on dynein activity , supporting previous evidence that She1 inhibits dynein .
	manualset3
99912	5	401127	13	NULL	NULL	0	NULL	dynein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased rates of detachment depend on dynein activity , supporting previous evidence that She1 inhibits dynein .
	manualset3
99913	1	401128	13	NULL	NULL	0	NULL	2 kb	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 kb ) contains regions necessary for tissue-specific expression and also a GC rich region which is essential for basal transcriptional activity .
	manualset3
99914	2	401128	13	NULL	NULL	0	NULL	regions 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	2 kb ) contains regions necessary for tissue-specific expression and also a GC rich region which is essential for basal transcriptional activity .
	manualset3
99915	3	401128	13	NULL	NULL	0	NULL	tissue-specific expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	2 kb ) contains regions necessary for tissue-specific expression and also a GC rich region which is essential for basal transcriptional activity .
	manualset3
99916	4	401128	13	NULL	NULL	0	NULL	GC rich region 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	2 kb ) contains regions necessary for tissue-specific expression and also a GC rich region which is essential for basal transcriptional activity .
	manualset3
99917	5	401128	13	NULL	NULL	0	NULL	basal transcriptional activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	2 kb ) contains regions necessary for tissue-specific expression and also a GC rich region which is essential for basal transcriptional activity .
	manualset3
99918	1	401129	13	NULL	NULL	0	NULL	serum ferritin concentrations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased serum ferritin concentrations in nonpathologic conditions , reflecting subclinical iron overload , have been reported to be associated with insulin resistance and an increased risk of type 2 diabetes mellitus ( DM ) .
	manualset3
99919	2	401129	13	NULL	NULL	0	NULL	nonpathologic conditions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased serum ferritin concentrations in nonpathologic conditions , reflecting subclinical iron overload , have been reported to be associated with insulin resistance and an increased risk of type 2 diabetes mellitus ( DM ) .
	manualset3
99920	3	401129	13	NULL	NULL	0	NULL	iron overload	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased serum ferritin concentrations in nonpathologic conditions , reflecting subclinical iron overload , have been reported to be associated with insulin resistance and an increased risk of type 2 diabetes mellitus ( DM ) .
	manualset3
99921	4	401129	13	NULL	NULL	0	NULL	insulin resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased serum ferritin concentrations in nonpathologic conditions , reflecting subclinical iron overload , have been reported to be associated with insulin resistance and an increased risk of type 2 diabetes mellitus ( DM ) .
	manualset3
99922	5	401129	13	NULL	NULL	0	NULL	risk of type 2 diabetes mellitus ( DM )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased serum ferritin concentrations in nonpathologic conditions , reflecting subclinical iron overload , have been reported to be associated with insulin resistance and an increased risk of type 2 diabetes mellitus ( DM ) .
	manualset3
99923	1	401130	13	NULL	NULL	0	NULL	tumor proliferation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased tumor proliferation and genomic instability without decreased apoptosis in MMTV-ras mice deficient in p53 .
	manualset3
99924	2	401130	13	NULL	NULL	0	NULL	genomic instability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased tumor proliferation and genomic instability without decreased apoptosis in MMTV-ras mice deficient in p53 .
	manualset3
99925	3	401130	13	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased tumor proliferation and genomic instability without decreased apoptosis in MMTV-ras mice deficient in p53 .
	manualset3
99926	4	401130	13	NULL	NULL	0	NULL	MMTV-ras mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased tumor proliferation and genomic instability without decreased apoptosis in MMTV-ras mice deficient in p53 .
	manualset3
99927	5	401130	13	NULL	NULL	0	NULL	p53	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased tumor proliferation and genomic instability without decreased apoptosis in MMTV-ras mice deficient in p53 .
	manualset3
100103	1	401131	13	NULL	NULL	0	NULL	vascular endothelial growth factor expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased vascular endothelial growth factor expression but impaired vascular endothelial growth factor receptor signaling in the myocardium of type 2 diabetic patients with chronic coronary heart disease .
	manualset3
100104	2	401131	13	NULL	NULL	0	NULL	vascular endothelial growth factor receptor signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased vascular endothelial growth factor expression but impaired vascular endothelial growth factor receptor signaling in the myocardium of type 2 diabetic patients with chronic coronary heart disease .
	manualset3
100105	3	401131	13	NULL	NULL	0	NULL	myocardium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased vascular endothelial growth factor expression but impaired vascular endothelial growth factor receptor signaling in the myocardium of type 2 diabetic patients with chronic coronary heart disease .
	manualset3
100106	4	401131	13	NULL	NULL	0	NULL	type 2 diabetic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased vascular endothelial growth factor expression but impaired vascular endothelial growth factor receptor signaling in the myocardium of type 2 diabetic patients with chronic coronary heart disease .
	manualset3
100107	5	401131	13	NULL	NULL	0	NULL	chronic coronary heart disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased vascular endothelial growth factor expression but impaired vascular endothelial growth factor receptor signaling in the myocardium of type 2 diabetic patients with chronic coronary heart disease .
	manualset3
100108	1	401132	13	NULL	NULL	0	NULL	extracellular potassium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Increases in extracellular potassium are considered to contribute to epileptogenesis , whereas adenosine has been proposed to be an endogenous antiepileptic agent .
	manualset3
100109	2	401132	13	NULL	NULL	0	NULL	epileptogenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increases in extracellular potassium are considered to contribute to epileptogenesis , whereas adenosine has been proposed to be an endogenous antiepileptic agent .
	manualset3
100110	3	401132	13	NULL	NULL	0	NULL	adenosine	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Increases in extracellular potassium are considered to contribute to epileptogenesis , whereas adenosine has been proposed to be an endogenous antiepileptic agent .
	manualset3
100111	4	401132	13	NULL	NULL	0	NULL	 antiepileptic agent 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Increases in extracellular potassium are considered to contribute to epileptogenesis , whereas adenosine has been proposed to be an endogenous antiepileptic agent .
	manualset3
100112	1	401133	13	NULL	NULL	0	NULL	concentrations 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing concentrations of Tween 20 resulted in greater amounts of extracted protein and lower cell viability .
	manualset3
100113	2	401133	13	NULL	NULL	0	NULL	Tween 20	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing concentrations of Tween 20 resulted in greater amounts of extracted protein and lower cell viability .
	manualset3
100114	3	401133	13	NULL	NULL	0	NULL	amounts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing concentrations of Tween 20 resulted in greater amounts of extracted protein and lower cell viability .
	manualset3
100115	4	401133	13	NULL	NULL	0	NULL	 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing concentrations of Tween 20 resulted in greater amounts of extracted protein and lower cell viability .
	manualset3
100116	5	401133	13	NULL	NULL	0	NULL	cell viability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing concentrations of Tween 20 resulted in greater amounts of extracted protein and lower cell viability .
	manualset3
100117	1	401134	13	NULL	NULL	0	NULL	correlation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing correlation length in bulk supercooled H2O , D2O , and NaCl solution determined from small angle x-ray scattering .
	manualset3
100118	2	401134	13	NULL	NULL	0	NULL	length	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing correlation length in bulk supercooled H2O , D2O , and NaCl solution determined from small angle x-ray scattering .
	manualset3
100119	3	401134	13	NULL	NULL	0	NULL	bulk	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing correlation length in bulk supercooled H2O , D2O , and NaCl solution determined from small angle x-ray scattering .
	manualset3
100120	4	401134	13	NULL	NULL	0	NULL	supercooled H2O	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing correlation length in bulk supercooled H2O , D2O , and NaCl solution determined from small angle x-ray scattering .
	manualset3
100121	5	401134	13	NULL	NULL	0	NULL	D2O	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing correlation length in bulk supercooled H2O , D2O , and NaCl solution determined from small angle x-ray scattering .
	manualset3
100122	6	401134	13	NULL	NULL	0	NULL	NaCl solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing correlation length in bulk supercooled H2O , D2O , and NaCl solution determined from small angle x-ray scattering .
	manualset3
100123	7	401134	13	NULL	NULL	0	NULL	small angle x-ray scattering 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing correlation length in bulk supercooled H2O , D2O , and NaCl solution determined from small angle x-ray scattering .
	manualset3
100124	1	401135	13	NULL	NULL	0	NULL	dermal perfusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing dermal perfusion after burning by decreasing thromboxane production .
	manualset3
100125	2	401135	13	NULL	NULL	0	NULL	thromboxane production 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing dermal perfusion after burning by decreasing thromboxane production .
	manualset3
100126	1	401136	13	NULL	NULL	0	NULL	doses of tyramine	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing doses of tyramine produced pressor effects which , in contrast to those of norepinephrine , were significantly attenuated by pre-treatment with L-NNA .
	manualset3
100127	2	401136	13	NULL	NULL	0	NULL	pressor effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing doses of tyramine produced pressor effects which , in contrast to those of norepinephrine , were significantly attenuated by pre-treatment with L-NNA .
	manualset3
100128	3	401136	13	NULL	NULL	0	NULL	norepinephrine 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing doses of tyramine produced pressor effects which , in contrast to those of norepinephrine , were significantly attenuated by pre-treatment with L-NNA .
	manualset3
100129	4	401136	13	NULL	NULL	0	NULL	 pre-treatment with L-NNA	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing doses of tyramine produced pressor effects which , in contrast to those of norepinephrine , were significantly attenuated by pre-treatment with L-NNA .
	manualset3
100130	1	401137	13	NULL	NULL	0	NULL	levels of CEA	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing levels of CEA were found in advanced stages of the disease .
	manualset3
100131	2	401137	13	NULL	NULL	0	NULL	advanced stages 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing levels of CEA were found in advanced stages of the disease .
	manualset3
100132	3	401137	13	NULL	NULL	0	NULL	 disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing levels of CEA were found in advanced stages of the disease .
	manualset3
100133	1	401138	13	NULL	NULL	0	NULL	 lipid peroxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing lipid peroxidation and trace element accumulation was observed with the use of an oxygen enriched aeration source .
	manualset3
100134	2	401138	13	NULL	NULL	0	NULL	trace element	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing lipid peroxidation and trace element accumulation was observed with the use of an oxygen enriched aeration source .
	manualset3
100136	3	401138	13	NULL	NULL	NULL	NULL	 accumulation 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Increasing lipid peroxidation and trace element accumulation was observed with the use of an oxygen enriched aeration source .
	manualset3
100137	4	401138	13	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing lipid peroxidation and trace element accumulation was observed with the use of an oxygen enriched aeration source .
	manualset3
100138	5	401138	13	NULL	NULL	0	NULL	oxygen enriched aeration source	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing lipid peroxidation and trace element accumulation was observed with the use of an oxygen enriched aeration source .
	manualset3
100139	1	401139	13	NULL	NULL	0	NULL	 medium Mg + + 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing medium Mg + + , prior to ischemia , to levels that greatly reduce energy requirements caused a significant improvement in the recovery of 2-deoxyglucose uptake .
	manualset3
100140	2	401139	13	NULL	NULL	0	NULL	ischemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing medium Mg + + , prior to ischemia , to levels that greatly reduce energy requirements caused a significant improvement in the recovery of 2-deoxyglucose uptake .
	manualset3
100141	3	401139	13	NULL	NULL	0	NULL	levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing medium Mg + + , prior to ischemia , to levels that greatly reduce energy requirements caused a significant improvement in the recovery of 2-deoxyglucose uptake .
	manualset3
100142	4	401139	13	NULL	NULL	0	NULL	energy requirements 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing medium Mg + + , prior to ischemia , to levels that greatly reduce energy requirements caused a significant improvement in the recovery of 2-deoxyglucose uptake .
	manualset3
100143	5	401139	13	NULL	NULL	0	NULL	improvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing medium Mg + + , prior to ischemia , to levels that greatly reduce energy requirements caused a significant improvement in the recovery of 2-deoxyglucose uptake .
	manualset3
100144	6	401139	13	NULL	NULL	0	NULL	recovery	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing medium Mg + + , prior to ischemia , to levels that greatly reduce energy requirements caused a significant improvement in the recovery of 2-deoxyglucose uptake .
	manualset3
100145	7	401139	13	NULL	NULL	0	NULL	2-deoxyglucose uptake	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing medium Mg + + , prior to ischemia , to levels that greatly reduce energy requirements caused a significant improvement in the recovery of 2-deoxyglucose uptake .
	manualset3
100146	1	401140	13	NULL	NULL	NULL	NULL	( K + )	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Increasing the ( K + ) o e-fold ( from 2.5 to 6.8 mM ) shifted the reversal potential of the GABAB current from -97.9 to -73.2 mV , as predicted by the Nernst equation .
	manualset3
100147	2	401140	13	NULL	NULL	0	NULL	o e-fold ( from 2.5 to 6.8 mM )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the ( K + ) o e-fold ( from 2.5 to 6.8 mM ) shifted the reversal potential of the GABAB current from -97.9 to -73.2 mV , as predicted by the Nernst equation .
	manualset3
100148	3	401140	13	NULL	NULL	0	NULL	reversal potential 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the ( K + ) o e-fold ( from 2.5 to 6.8 mM ) shifted the reversal potential of the GABAB current from -97.9 to -73.2 mV , as predicted by the Nernst equation .
	manualset3
100149	4	401140	13	NULL	NULL	0	NULL	GABAB current	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the ( K + ) o e-fold ( from 2.5 to 6.8 mM ) shifted the reversal potential of the GABAB current from -97.9 to -73.2 mV , as predicted by the Nernst equation .
	manualset3
100150	5	401140	13	NULL	NULL	0	NULL	from -97.9 to -73.2 mV	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the ( K + ) o e-fold ( from 2.5 to 6.8 mM ) shifted the reversal potential of the GABAB current from -97.9 to -73.2 mV , as predicted by the Nernst equation .
	manualset3
100151	6	401140	13	NULL	NULL	0	NULL	Nernst equation	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the ( K + ) o e-fold ( from 2.5 to 6.8 mM ) shifted the reversal potential of the GABAB current from -97.9 to -73.2 mV , as predicted by the Nernst equation .
	manualset3
100152	1	401141	13	NULL	NULL	0	NULL	MgATP concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the MgATP concentration shifts the pCa - % maximum tension relationship in the direction of increasing Ca required for activation .
	manualset3
100153	2	401141	13	NULL	NULL	0	NULL	pCa - % maximum tension relationship	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the MgATP concentration shifts the pCa - % maximum tension relationship in the direction of increasing Ca required for activation .
	manualset3
100154	3	401141	13	NULL	NULL	0	NULL	direction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the MgATP concentration shifts the pCa - % maximum tension relationship in the direction of increasing Ca required for activation .
	manualset3
100155	4	401141	13	NULL	NULL	0	NULL	Ca	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the MgATP concentration shifts the pCa - % maximum tension relationship in the direction of increasing Ca required for activation .
	manualset3
100156	5	401141	13	NULL	NULL	0	NULL	activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the MgATP concentration shifts the pCa - % maximum tension relationship in the direction of increasing Ca required for activation .
	manualset3
100157	1	401142	13	NULL	NULL	0	NULL	dosage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the dosage of DNA or chromosomes resulted in an almost linear increase in the number of transformants .
	manualset3
100158	2	401142	13	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the dosage of DNA or chromosomes resulted in an almost linear increase in the number of transformants .
	manualset3
100159	3	401142	13	NULL	NULL	0	NULL	chromosomes	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the dosage of DNA or chromosomes resulted in an almost linear increase in the number of transformants .
	manualset3
100160	4	401142	13	NULL	NULL	0	NULL	 linear increase	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the dosage of DNA or chromosomes resulted in an almost linear increase in the number of transformants .
	manualset3
100161	5	401142	13	NULL	NULL	0	NULL	number of transformants	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the dosage of DNA or chromosomes resulted in an almost linear increase in the number of transformants .
	manualset3
100162	1	401143	13	NULL	NULL	0	NULL	duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the duration of the TCDD exposure prior to its withdrawal led to an increased AHF size , phenotypic complexity and number of AHF remaining after cessation of TCDD administration .
	manualset3
100163	2	401143	13	NULL	NULL	0	NULL	TCDD exposure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the duration of the TCDD exposure prior to its withdrawal led to an increased AHF size , phenotypic complexity and number of AHF remaining after cessation of TCDD administration .
	manualset3
100164	3	401143	13	NULL	NULL	0	NULL	withdrawal	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the duration of the TCDD exposure prior to its withdrawal led to an increased AHF size , phenotypic complexity and number of AHF remaining after cessation of TCDD administration .
	manualset3
100165	4	401143	13	NULL	NULL	0	NULL	 AHF size	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the duration of the TCDD exposure prior to its withdrawal led to an increased AHF size , phenotypic complexity and number of AHF remaining after cessation of TCDD administration .
	manualset3
100166	5	401143	13	NULL	NULL	0	NULL	phenotypic complexity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the duration of the TCDD exposure prior to its withdrawal led to an increased AHF size , phenotypic complexity and number of AHF remaining after cessation of TCDD administration .
	manualset3
100167	6	401143	13	NULL	NULL	0	NULL	number of AHF	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the duration of the TCDD exposure prior to its withdrawal led to an increased AHF size , phenotypic complexity and number of AHF remaining after cessation of TCDD administration .
	manualset3
100168	7	401143	13	NULL	NULL	0	NULL	cessation of TCDD 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the duration of the TCDD exposure prior to its withdrawal led to an increased AHF size , phenotypic complexity and number of AHF remaining after cessation of TCDD administration .
	manualset3
100169	1	401144	13	NULL	NULL	0	NULL	inositol concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the inositol concentration in the medium to 300 microM produced a 14-fold stimulation of phosphatidylinositol synthesis but only a 5-fold increase in phosphatidylinositol 4 , 5-bisphosphate synthesis .
	manualset3
100170	2	401144	13	NULL	NULL	0	NULL	medium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the inositol concentration in the medium to 300 microM produced a 14-fold stimulation of phosphatidylinositol synthesis but only a 5-fold increase in phosphatidylinositol 4 , 5-bisphosphate synthesis .
	manualset3
100171	3	401144	13	NULL	NULL	0	NULL	300 microM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the inositol concentration in the medium to 300 microM produced a 14-fold stimulation of phosphatidylinositol synthesis but only a 5-fold increase in phosphatidylinositol 4 , 5-bisphosphate synthesis .
	manualset3
100172	4	401144	13	NULL	NULL	NULL	NULL	14-fold stimulation 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Increasing the inositol concentration in the medium to 300 microM produced a 14-fold stimulation of phosphatidylinositol synthesis but only a 5-fold increase in phosphatidylinositol 4 , 5-bisphosphate synthesis .
	manualset3
100173	5	401144	13	NULL	NULL	0	NULL	phosphatidylinositol synthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the inositol concentration in the medium to 300 microM produced a 14-fold stimulation of phosphatidylinositol synthesis but only a 5-fold increase in phosphatidylinositol 4 , 5-bisphosphate synthesis .
	manualset3
100174	6	401144	13	NULL	NULL	0	NULL	5-fold increase	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the inositol concentration in the medium to 300 microM produced a 14-fold stimulation of phosphatidylinositol synthesis but only a 5-fold increase in phosphatidylinositol 4 , 5-bisphosphate synthesis .
	manualset3
100175	7	401144	13	NULL	NULL	0	NULL	phosphatidylinositol 4 , 5-bisphosphate synthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the inositol concentration in the medium to 300 microM produced a 14-fold stimulation of phosphatidylinositol synthesis but only a 5-fold increase in phosphatidylinositol 4 , 5-bisphosphate synthesis .
	manualset3
100176	1	401145	13	NULL	NULL	0	NULL	level of the MT antigen	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the level of the MT antigen led to increased expression of transformation , assayed by morphology , focus formation and growth in agar .
	manualset3
100177	2	401145	13	NULL	NULL	0	NULL	expression of transformation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the level of the MT antigen led to increased expression of transformation , assayed by morphology , focus formation and growth in agar .
	manualset3
100178	3	401145	13	NULL	NULL	0	NULL	morphology 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the level of the MT antigen led to increased expression of transformation , assayed by morphology , focus formation and growth in agar .
	manualset3
100179	4	401145	13	NULL	NULL	0	NULL	focus formation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the level of the MT antigen led to increased expression of transformation , assayed by morphology , focus formation and growth in agar .
	manualset3
100180	5	401145	13	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the level of the MT antigen led to increased expression of transformation , assayed by morphology , focus formation and growth in agar .
	manualset3
100181	6	401145	13	NULL	NULL	0	NULL	agar	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the level of the MT antigen led to increased expression of transformation , assayed by morphology , focus formation and growth in agar .
	manualset3
100182	1	401146	13	NULL	NULL	NULL	NULL	validity	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Increasing the validity of research results with a blend of laboratory and clinical strategies .
	manualset3
100183	2	401146	13	NULL	NULL	0	NULL	research results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the validity of research results with a blend of laboratory and clinical strategies .
	manualset3
100184	3	401146	13	NULL	NULL	0	NULL	blend	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the validity of research results with a blend of laboratory and clinical strategies .
	manualset3
100185	4	401146	13	NULL	NULL	0	NULL	 laboratory strategies	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the validity of research results with a blend of laboratory and clinical strategies .
	manualset3
100186	5	401146	13	NULL	NULL	0	NULL	 clinical strategies	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Increasing the validity of research results with a blend of laboratory and clinical strategies .
	manualset3
100187	1	401147	13	NULL	NULL	0	NULL	20 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	20 % by day 16 , while component EII increases in an inverse manner to that of component EI .
	manualset3
100188	2	401147	13	NULL	NULL	0	NULL	 day 16	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	20 % by day 16 , while component EII increases in an inverse manner to that of component EI .
	manualset3
100189	3	401147	13	NULL	NULL	0	NULL	 component EII	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	20 % by day 16 , while component EII increases in an inverse manner to that of component EI .
	manualset3
100191	5	401147	13	NULL	NULL	0	NULL	inverse manner	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	20 % by day 16 , while component EII increases in an inverse manner to that of component EI .
	manualset3
100192	6	401147	13	NULL	NULL	0	NULL	component EI 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	20 % by day 16 , while component EII increases in an inverse manner to that of component EI .
	manualset3
100193	1	401148	13	NULL	NULL	0	NULL	female emperor geese 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubating female emperor geese had high selenium concentrations in their blood , accompanied by increased glutathione peroxidase activity consistent with early oxidative stress .
	manualset3
100194	2	401148	13	NULL	NULL	0	NULL	high selenium concentrations 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubating female emperor geese had high selenium concentrations in their blood , accompanied by increased glutathione peroxidase activity consistent with early oxidative stress .
	manualset3
100195	3	401148	13	NULL	NULL	0	NULL	blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubating female emperor geese had high selenium concentrations in their blood , accompanied by increased glutathione peroxidase activity consistent with early oxidative stress .
	manualset3
100196	4	401148	13	NULL	NULL	0	NULL	glutathione peroxidase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubating female emperor geese had high selenium concentrations in their blood , accompanied by increased glutathione peroxidase activity consistent with early oxidative stress .
	manualset3
100197	5	401148	13	NULL	NULL	0	NULL	oxidative stress	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubating female emperor geese had high selenium concentrations in their blood , accompanied by increased glutathione peroxidase activity consistent with early oxidative stress .
	manualset3
100198	1	401149	13	NULL	NULL	0	NULL	Incubation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubation of FRTL5 cells with TSH induced a time - and concentration-dependent increase in GLUT1 mRNA levels , while GLUT4 mRNA levels were decreased .
	manualset3
100199	2	401149	13	NULL	NULL	0	NULL	FRTL5 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubation of FRTL5 cells with TSH induced a time - and concentration-dependent increase in GLUT1 mRNA levels , while GLUT4 mRNA levels were decreased .
	manualset3
100200	3	401149	13	NULL	NULL	0	NULL	TSH	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubation of FRTL5 cells with TSH induced a time - and concentration-dependent increase in GLUT1 mRNA levels , while GLUT4 mRNA levels were decreased .
	manualset3
100201	4	401149	13	NULL	NULL	NULL	NULL	time-dependent increase	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Incubation of FRTL5 cells with TSH induced a time - and concentration-dependent increase in GLUT1 mRNA levels , while GLUT4 mRNA levels were decreased .
	manualset3
100202	5	401149	13	NULL	NULL	0	NULL	concentration-dependent increase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubation of FRTL5 cells with TSH induced a time - and concentration-dependent increase in GLUT1 mRNA levels , while GLUT4 mRNA levels were decreased .
	manualset3
100203	6	401149	13	NULL	NULL	NULL	NULL	GLUT1 mRNA levels	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Incubation of FRTL5 cells with TSH induced a time - and concentration-dependent increase in GLUT1 mRNA levels , while GLUT4 mRNA levels were decreased .
	manualset3
100204	7	401149	13	NULL	NULL	0	NULL	GLUT4 mRNA levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubation of FRTL5 cells with TSH induced a time - and concentration-dependent increase in GLUT1 mRNA levels , while GLUT4 mRNA levels were decreased .
	manualset3
100205	1	401150	13	NULL	NULL	0	NULL	Incubation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubation of lymphoblasts with isoprenaline ( 1 nM ) for 24 h prior to assay reduced both receptor number and adenylyl cyclase activity .
	manualset3
100206	2	401150	13	NULL	NULL	0	NULL	lymphoblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubation of lymphoblasts with isoprenaline ( 1 nM ) for 24 h prior to assay reduced both receptor number and adenylyl cyclase activity .
	manualset3
100207	3	401150	13	NULL	NULL	0	NULL	isoprenaline ( 1 nM )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubation of lymphoblasts with isoprenaline ( 1 nM ) for 24 h prior to assay reduced both receptor number and adenylyl cyclase activity .
	manualset3
100208	4	401150	13	NULL	NULL	0	NULL	24 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubation of lymphoblasts with isoprenaline ( 1 nM ) for 24 h prior to assay reduced both receptor number and adenylyl cyclase activity .
	manualset3
100209	5	401150	13	NULL	NULL	0	NULL	assay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubation of lymphoblasts with isoprenaline ( 1 nM ) for 24 h prior to assay reduced both receptor number and adenylyl cyclase activity .
	manualset3
100210	6	401150	13	NULL	NULL	0	NULL	receptor number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubation of lymphoblasts with isoprenaline ( 1 nM ) for 24 h prior to assay reduced both receptor number and adenylyl cyclase activity .
	manualset3
100211	7	401150	13	NULL	NULL	0	NULL	adenylyl cyclase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubation of lymphoblasts with isoprenaline ( 1 nM ) for 24 h prior to assay reduced both receptor number and adenylyl cyclase activity .
	manualset3
100212	1	401151	13	NULL	NULL	0	NULL	Incubation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubation of these cells with p-nitrophenylxyloside , known to inhibit proteoglycan formation , also increased this nonamyloidogenic cleavage of APP .
	manualset3
100213	2	401151	13	NULL	NULL	0	NULL	 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubation of these cells with p-nitrophenylxyloside , known to inhibit proteoglycan formation , also increased this nonamyloidogenic cleavage of APP .
	manualset3
100214	3	401151	13	NULL	NULL	0	NULL	p-nitrophenylxyloside	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubation of these cells with p-nitrophenylxyloside , known to inhibit proteoglycan formation , also increased this nonamyloidogenic cleavage of APP .
	manualset3
100215	4	401151	13	NULL	NULL	0	NULL	proteoglycan formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubation of these cells with p-nitrophenylxyloside , known to inhibit proteoglycan formation , also increased this nonamyloidogenic cleavage of APP .
	manualset3
100216	5	401151	13	NULL	NULL	0	NULL	nonamyloidogenic cleavage 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubation of these cells with p-nitrophenylxyloside , known to inhibit proteoglycan formation , also increased this nonamyloidogenic cleavage of APP .
	manualset3
100217	6	401151	13	NULL	NULL	0	NULL	APP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubation of these cells with p-nitrophenylxyloside , known to inhibit proteoglycan formation , also increased this nonamyloidogenic cleavage of APP .
	manualset3
100218	1	401152	13	NULL	NULL	0	NULL	Incubation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubation with 17beta-estradiol enhanced relaxations to bradykinin ( from 43 + / - 6 to 83 + / - 3 % , P & lt ; 0.0001 ) but not those to nitroglycerine ( n.s. ) .
	manualset3
100219	2	401152	13	NULL	NULL	0	NULL	17beta-estradiol 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubation with 17beta-estradiol enhanced relaxations to bradykinin ( from 43 + / - 6 to 83 + / - 3 % , P & lt ; 0.0001 ) but not those to nitroglycerine ( n.s. ) .
	manualset3
100220	3	401152	13	NULL	NULL	0	NULL	relaxations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubation with 17beta-estradiol enhanced relaxations to bradykinin ( from 43 + / - 6 to 83 + / - 3 % , P & lt ; 0.0001 ) but not those to nitroglycerine ( n.s. ) .
	manualset3
100221	4	401152	13	NULL	NULL	0	NULL	bradykinin	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubation with 17beta-estradiol enhanced relaxations to bradykinin ( from 43 + / - 6 to 83 + / - 3 % , P & lt ; 0.0001 ) but not those to nitroglycerine ( n.s. ) .
	manualset3
100222	5	401152	13	NULL	NULL	0	NULL	rom 43 + / - 6 to 83 + / - 3 % , P & lt ; 0.0001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubation with 17beta-estradiol enhanced relaxations to bradykinin ( from 43 + / - 6 to 83 + / - 3 % , P & lt ; 0.0001 ) but not those to nitroglycerine ( n.s. ) .
	manualset3
100223	6	401152	13	NULL	NULL	0	NULL	nitroglycerine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubation with 17beta-estradiol enhanced relaxations to bradykinin ( from 43 + / - 6 to 83 + / - 3 % , P & lt ; 0.0001 ) but not those to nitroglycerine ( n.s. ) .
	manualset3
100224	1	401153	13	NULL	NULL	0	NULL	variety of complex liver diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , a variety of complex liver diseases can lead to decreased synthesis of the same set of coagulation factors as in hemophilia .
	manualset3
100225	2	401153	13	NULL	NULL	0	NULL	synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , a variety of complex liver diseases can lead to decreased synthesis of the same set of coagulation factors as in hemophilia .
	manualset3
100226	3	401153	13	NULL	NULL	0	NULL	set of coagulation factors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , a variety of complex liver diseases can lead to decreased synthesis of the same set of coagulation factors as in hemophilia .
	manualset3
100227	4	401153	13	NULL	NULL	0	NULL	hemophilia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , a variety of complex liver diseases can lead to decreased synthesis of the same set of coagulation factors as in hemophilia .
	manualset3
100228	1	401154	13	NULL	NULL	0	NULL	acute infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , acute infection in this model is characterized by high rates of viral replication associated with early cytokine dysregulations , in the absence of opportunistic infection .
	manualset3
100229	2	401154	13	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , acute infection in this model is characterized by high rates of viral replication associated with early cytokine dysregulations , in the absence of opportunistic infection .
	manualset3
100230	3	401154	13	NULL	NULL	0	NULL	high rates	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , acute infection in this model is characterized by high rates of viral replication associated with early cytokine dysregulations , in the absence of opportunistic infection .
	manualset3
100231	4	401154	13	NULL	NULL	0	NULL	viral replication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , acute infection in this model is characterized by high rates of viral replication associated with early cytokine dysregulations , in the absence of opportunistic infection .
	manualset3
100232	5	401154	13	NULL	NULL	0	NULL	cytokine dysregulations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , acute infection in this model is characterized by high rates of viral replication associated with early cytokine dysregulations , in the absence of opportunistic infection .
	manualset3
100233	6	401154	13	NULL	NULL	0	NULL	absence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , acute infection in this model is characterized by high rates of viral replication associated with early cytokine dysregulations , in the absence of opportunistic infection .
	manualset3
100234	7	401154	13	NULL	NULL	0	NULL	opportunistic infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , acute infection in this model is characterized by high rates of viral replication associated with early cytokine dysregulations , in the absence of opportunistic infection .
	manualset3
100235	1	401155	13	NULL	NULL	0	NULL	bile acids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , bile acids strongly bind to circulating albumin : consequently ascitic fluid contains more cholic acid ( less hydrophobic ) than other bile acids .
	manualset3
100236	2	401155	13	NULL	NULL	0	NULL	albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , bile acids strongly bind to circulating albumin : consequently ascitic fluid contains more cholic acid ( less hydrophobic ) than other bile acids .
	manualset3
100237	3	401155	13	NULL	NULL	0	NULL	ascitic fluid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , bile acids strongly bind to circulating albumin : consequently ascitic fluid contains more cholic acid ( less hydrophobic ) than other bile acids .
	manualset3
100238	4	401155	13	NULL	NULL	0	NULL	cholic acid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , bile acids strongly bind to circulating albumin : consequently ascitic fluid contains more cholic acid ( less hydrophobic ) than other bile acids .
	manualset3
100239	5	401155	13	NULL	NULL	0	NULL	bile acids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , bile acids strongly bind to circulating albumin : consequently ascitic fluid contains more cholic acid ( less hydrophobic ) than other bile acids .
	manualset3
100240	1	401156	13	NULL	NULL	0	NULL	recent data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , recent data from different research groups have highlighted the anti-HIV activity of some DING representatives .
	manualset3
100241	2	401156	13	NULL	NULL	0	NULL	research groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , recent data from different research groups have highlighted the anti-HIV activity of some DING representatives .
	manualset3
100242	3	401156	13	NULL	NULL	0	NULL	anti-HIV activity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , recent data from different research groups have highlighted the anti-HIV activity of some DING representatives .
	manualset3
100243	4	401156	13	NULL	NULL	0	NULL	DING representatives	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , recent data from different research groups have highlighted the anti-HIV activity of some DING representatives .
	manualset3
100244	1	401157	13	NULL	NULL	0	NULL	early 1980s	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , since the early 1980s , the accumulating knowledge of the endothelial cell structure as well as of the functional properties of the endothelial cells shifted their role from a passive membrane or barrier to a complex tissue with complex functions adaptable to needs specific in time and location .
	manualset3
100245	2	401157	13	NULL	NULL	0	NULL	 knowledge	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , since the early 1980s , the accumulating knowledge of the endothelial cell structure as well as of the functional properties of the endothelial cells shifted their role from a passive membrane or barrier to a complex tissue with complex functions adaptable to needs specific in time and location .
	manualset3
100246	3	401157	13	NULL	NULL	0	NULL	endothelial cell structure	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , since the early 1980s , the accumulating knowledge of the endothelial cell structure as well as of the functional properties of the endothelial cells shifted their role from a passive membrane or barrier to a complex tissue with complex functions adaptable to needs specific in time and location .
	manualset3
100247	4	401157	13	NULL	NULL	0	NULL	functional properties	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , since the early 1980s , the accumulating knowledge of the endothelial cell structure as well as of the functional properties of the endothelial cells shifted their role from a passive membrane or barrier to a complex tissue with complex functions adaptable to needs specific in time and location .
	manualset3
100248	5	401157	13	NULL	NULL	0	NULL	 endothelial cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , since the early 1980s , the accumulating knowledge of the endothelial cell structure as well as of the functional properties of the endothelial cells shifted their role from a passive membrane or barrier to a complex tissue with complex functions adaptable to needs specific in time and location .
	manualset3
100250	6	401157	13	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , since the early 1980s , the accumulating knowledge of the endothelial cell structure as well as of the functional properties of the endothelial cells shifted their role from a passive membrane or barrier to a complex tissue with complex functions adaptable to needs specific in time and location .
	manualset3
100251	7	401157	13	NULL	NULL	0	NULL	passive membrane 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , since the early 1980s , the accumulating knowledge of the endothelial cell structure as well as of the functional properties of the endothelial cells shifted their role from a passive membrane or barrier to a complex tissue with complex functions adaptable to needs specific in time and location .
	manualset3
100252	8	401157	13	NULL	NULL	0	NULL	barrier	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , since the early 1980s , the accumulating knowledge of the endothelial cell structure as well as of the functional properties of the endothelial cells shifted their role from a passive membrane or barrier to a complex tissue with complex functions adaptable to needs specific in time and location .
	manualset3
100253	9	401157	13	NULL	NULL	0	NULL	complex tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , since the early 1980s , the accumulating knowledge of the endothelial cell structure as well as of the functional properties of the endothelial cells shifted their role from a passive membrane or barrier to a complex tissue with complex functions adaptable to needs specific in time and location .
	manualset3
100254	10	401157	13	NULL	NULL	0	NULL	complex functions 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , since the early 1980s , the accumulating knowledge of the endothelial cell structure as well as of the functional properties of the endothelial cells shifted their role from a passive membrane or barrier to a complex tissue with complex functions adaptable to needs specific in time and location .
	manualset3
100255	11	401157	13	NULL	NULL	0	NULL	needs	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , since the early 1980s , the accumulating knowledge of the endothelial cell structure as well as of the functional properties of the endothelial cells shifted their role from a passive membrane or barrier to a complex tissue with complex functions adaptable to needs specific in time and location .
	manualset3
100256	12	401157	13	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , since the early 1980s , the accumulating knowledge of the endothelial cell structure as well as of the functional properties of the endothelial cells shifted their role from a passive membrane or barrier to a complex tissue with complex functions adaptable to needs specific in time and location .
	manualset3
100257	13	401157	13	NULL	NULL	0	NULL	location 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , since the early 1980s , the accumulating knowledge of the endothelial cell structure as well as of the functional properties of the endothelial cells shifted their role from a passive membrane or barrier to a complex tissue with complex functions adaptable to needs specific in time and location .
	manualset3
100258	1	401158	13	NULL	NULL	0	NULL	 use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , the use of a non-synonymous to synonymous substitution rate ratio parameter has facilitated the interpretation of selection pressure on genomes .
	manualset3
100259	2	401158	13	NULL	NULL	NULL	NULL	non-synonymous to synonymous substitution rate ratio parameter	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Indeed , the use of a non-synonymous to synonymous substitution rate ratio parameter has facilitated the interpretation of selection pressure on genomes .
	manualset3
100260	3	401158	13	NULL	NULL	0	NULL	 interpretation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , the use of a non-synonymous to synonymous substitution rate ratio parameter has facilitated the interpretation of selection pressure on genomes .
	manualset3
100261	4	401158	13	NULL	NULL	0	NULL	selection pressure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , the use of a non-synonymous to synonymous substitution rate ratio parameter has facilitated the interpretation of selection pressure on genomes .
	manualset3
100262	5	401158	13	NULL	NULL	0	NULL	genomes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , the use of a non-synonymous to synonymous substitution rate ratio parameter has facilitated the interpretation of selection pressure on genomes .
	manualset3
100263	1	401159	13	NULL	NULL	0	NULL	transsexual women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , transsexual women ( male-to-female transsexual patients ) may be given the option to store spermatozoa before they start hormonal therapy , so that their gametes may be used in future relationships .
	manualset3
100264	2	401159	13	NULL	NULL	0	NULL	male-to-female transsexual patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , transsexual women ( male-to-female transsexual patients ) may be given the option to store spermatozoa before they start hormonal therapy , so that their gametes may be used in future relationships .
	manualset3
100265	3	401159	13	NULL	NULL	0	NULL	option	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , transsexual women ( male-to-female transsexual patients ) may be given the option to store spermatozoa before they start hormonal therapy , so that their gametes may be used in future relationships .
	manualset3
100266	4	401159	13	NULL	NULL	0	NULL	 spermatozoa	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , transsexual women ( male-to-female transsexual patients ) may be given the option to store spermatozoa before they start hormonal therapy , so that their gametes may be used in future relationships .
	manualset3
100267	5	401159	13	NULL	NULL	0	NULL	hormonal therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , transsexual women ( male-to-female transsexual patients ) may be given the option to store spermatozoa before they start hormonal therapy , so that their gametes may be used in future relationships .
	manualset3
100268	6	401159	13	NULL	NULL	0	NULL	gametes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , transsexual women ( male-to-female transsexual patients ) may be given the option to store spermatozoa before they start hormonal therapy , so that their gametes may be used in future relationships .
	manualset3
100269	7	401159	13	NULL	NULL	0	NULL	future	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , transsexual women ( male-to-female transsexual patients ) may be given the option to store spermatozoa before they start hormonal therapy , so that their gametes may be used in future relationships .
	manualset3
100270	8	401159	13	NULL	NULL	0	NULL	relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , transsexual women ( male-to-female transsexual patients ) may be given the option to store spermatozoa before they start hormonal therapy , so that their gametes may be used in future relationships .
	manualset3
100271	1	401160	13	NULL	NULL	0	NULL	possibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , we may view the possibility of linking human electromagnetic interactions with mechanical vibrations of the crystalline lattices of genes and associated critical molecules like growth factors .
	manualset3
100272	2	401160	13	NULL	NULL	0	NULL	human electromagnetic interactions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , we may view the possibility of linking human electromagnetic interactions with mechanical vibrations of the crystalline lattices of genes and associated critical molecules like growth factors .
	manualset3
100273	3	401160	13	NULL	NULL	0	NULL	mechanical vibrations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , we may view the possibility of linking human electromagnetic interactions with mechanical vibrations of the crystalline lattices of genes and associated critical molecules like growth factors .
	manualset3
100274	4	401160	13	NULL	NULL	0	NULL	crystalline lattices of genes	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , we may view the possibility of linking human electromagnetic interactions with mechanical vibrations of the crystalline lattices of genes and associated critical molecules like growth factors .
	manualset3
100275	5	401160	13	NULL	NULL	0	NULL	critical molecules	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , we may view the possibility of linking human electromagnetic interactions with mechanical vibrations of the crystalline lattices of genes and associated critical molecules like growth factors .
	manualset3
100276	6	401160	13	NULL	NULL	0	NULL	growth factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , we may view the possibility of linking human electromagnetic interactions with mechanical vibrations of the crystalline lattices of genes and associated critical molecules like growth factors .
	manualset3
100277	1	401161	13	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed application of PLS-DA to in vivo data allowed identification of a set of genes able to discriminate primary lung tumors from colon metastases .
	manualset3
100278	2	401161	13	NULL	NULL	0	NULL	PLS-DA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed application of PLS-DA to in vivo data allowed identification of a set of genes able to discriminate primary lung tumors from colon metastases .
	manualset3
100279	3	401161	13	NULL	NULL	0	NULL	in vivo data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed application of PLS-DA to in vivo data allowed identification of a set of genes able to discriminate primary lung tumors from colon metastases .
	manualset3
100280	4	401161	13	NULL	NULL	0	NULL	identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed application of PLS-DA to in vivo data allowed identification of a set of genes able to discriminate primary lung tumors from colon metastases .
	manualset3
100281	5	401161	13	NULL	NULL	0	NULL	set of genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed application of PLS-DA to in vivo data allowed identification of a set of genes able to discriminate primary lung tumors from colon metastases .
	manualset3
100282	6	401161	13	NULL	NULL	0	NULL	primary lung tumors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed application of PLS-DA to in vivo data allowed identification of a set of genes able to discriminate primary lung tumors from colon metastases .
	manualset3
100283	7	401161	13	NULL	NULL	0	NULL	colon metastases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed application of PLS-DA to in vivo data allowed identification of a set of genes able to discriminate primary lung tumors from colon metastases .
	manualset3
100284	1	401162	13	NULL	NULL	NULL	NULL	actual number 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Indeed since the actual number of intestinal infection related deaths did fall while the populations grew considerably , there was a true reduced risk of death from these infections .
	manualset3
100285	2	401162	13	NULL	NULL	0	NULL	intestinal infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed since the actual number of intestinal infection related deaths did fall while the populations grew considerably , there was a true reduced risk of death from these infections .
	manualset3
100286	3	401162	13	NULL	NULL	0	NULL	deaths	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed since the actual number of intestinal infection related deaths did fall while the populations grew considerably , there was a true reduced risk of death from these infections .
	manualset3
100288	5	401162	13	NULL	NULL	0	NULL	populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed since the actual number of intestinal infection related deaths did fall while the populations grew considerably , there was a true reduced risk of death from these infections .
	manualset3
100289	6	401162	13	NULL	NULL	0	NULL	risk of death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed since the actual number of intestinal infection related deaths did fall while the populations grew considerably , there was a true reduced risk of death from these infections .
	manualset3
100290	7	401162	13	NULL	NULL	0	NULL	infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed since the actual number of intestinal infection related deaths did fall while the populations grew considerably , there was a true reduced risk of death from these infections .
	manualset3
100292	1	401163	13	NULL	NULL	0	NULL	Indemnity insurance 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Indemnity insurance : an update .
	manualset3
100298	1	401164	13	NULL	NULL	NULL	NULL	Independence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Independence of the drug action of both the heart rate and the isoproterenol-induced changes in refractoriness are related to the ability of AL-275 to block a slow component ( IKs ) of the potassium current .
	manualset3
100299	2	401164	13	NULL	NULL	0	NULL	drug action	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Independence of the drug action of both the heart rate and the isoproterenol-induced changes in refractoriness are related to the ability of AL-275 to block a slow component ( IKs ) of the potassium current .
	manualset3
100300	3	401164	13	NULL	NULL	0	NULL	 heart rate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Independence of the drug action of both the heart rate and the isoproterenol-induced changes in refractoriness are related to the ability of AL-275 to block a slow component ( IKs ) of the potassium current .
	manualset3
100301	4	401164	13	NULL	NULL	0	NULL	isoproterenol-induced changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Independence of the drug action of both the heart rate and the isoproterenol-induced changes in refractoriness are related to the ability of AL-275 to block a slow component ( IKs ) of the potassium current .
	manualset3
100306	5	401164	13	NULL	NULL	0	NULL	refractoriness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Independence of the drug action of both the heart rate and the isoproterenol-induced changes in refractoriness are related to the ability of AL-275 to block a slow component ( IKs ) of the potassium current .
	manualset3
100308	6	401164	13	NULL	NULL	0	NULL	ability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Independence of the drug action of both the heart rate and the isoproterenol-induced changes in refractoriness are related to the ability of AL-275 to block a slow component ( IKs ) of the potassium current .
	manualset3
100312	7	401164	13	NULL	NULL	0	NULL	AL-275	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Independence of the drug action of both the heart rate and the isoproterenol-induced changes in refractoriness are related to the ability of AL-275 to block a slow component ( IKs ) of the potassium current .
	manualset3
100313	8	401164	13	NULL	NULL	0	NULL	component ( IKs ) of the potassium current	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Independence of the drug action of both the heart rate and the isoproterenol-induced changes in refractoriness are related to the ability of AL-275 to block a slow component ( IKs ) of the potassium current .
	manualset3
100317	2	401165	13	NULL	NULL	NULL	NULL	heat controls 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Independent heat controls for the water bath and the delivery tubing allow precision of humidities in the gases provided for inspiration through an artificial airway .
	manualset3
100318	3	401165	13	NULL	NULL	0	NULL	water bath	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Independent heat controls for the water bath and the delivery tubing allow precision of humidities in the gases provided for inspiration through an artificial airway .
	manualset3
100319	4	401165	13	NULL	NULL	0	NULL	delivery tubing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Independent heat controls for the water bath and the delivery tubing allow precision of humidities in the gases provided for inspiration through an artificial airway .
	manualset3
100322	5	401165	13	NULL	NULL	0	NULL	precision of humidities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Independent heat controls for the water bath and the delivery tubing allow precision of humidities in the gases provided for inspiration through an artificial airway .
	manualset3
100325	6	401165	13	NULL	NULL	0	NULL	 gases	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Independent heat controls for the water bath and the delivery tubing allow precision of humidities in the gases provided for inspiration through an artificial airway .
	manualset3
100327	7	401165	13	NULL	NULL	0	NULL	inspiration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Independent heat controls for the water bath and the delivery tubing allow precision of humidities in the gases provided for inspiration through an artificial airway .
	manualset3
100328	8	401165	13	NULL	NULL	0	NULL	artificial airway	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Independent heat controls for the water bath and the delivery tubing allow precision of humidities in the gases provided for inspiration through an artificial airway .
	manualset3
100330	1	401166	13	NULL	NULL	0	NULL	Independent origin	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Independent origin of multiple foci of prostatic intraepithelial neoplasia : comparison with matched foci of prostate carcinoma .
	manualset3
100331	2	401166	13	NULL	NULL	0	NULL	multiple foci of prostatic intraepithelial neoplasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Independent origin of multiple foci of prostatic intraepithelial neoplasia : comparison with matched foci of prostate carcinoma .
	manualset3
100333	3	401166	13	NULL	NULL	0	NULL	 comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Independent origin of multiple foci of prostatic intraepithelial neoplasia : comparison with matched foci of prostate carcinoma .
	manualset3
100334	4	401166	13	NULL	NULL	0	NULL	foci of prostate carcinoma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Independent origin of multiple foci of prostatic intraepithelial neoplasia : comparison with matched foci of prostate carcinoma .
	manualset3
100335	1	401167	13	NULL	NULL	0	NULL	Independent risk factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Independent risk factors identified were age 75 years , being a healthcare worker , and injecting drug use .
	manualset3
100336	2	401167	13	NULL	NULL	0	NULL	age 75 years	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Independent risk factors identified were age 75 years , being a healthcare worker , and injecting drug use .
	manualset3
100337	3	401167	13	NULL	NULL	0	NULL	healthcare worker	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Independent risk factors identified were age 75 years , being a healthcare worker , and injecting drug use .
	manualset3
100338	4	401167	13	NULL	NULL	0	NULL	drug use	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Independent risk factors identified were age 75 years , being a healthcare worker , and injecting drug use .
	manualset3
100339	1	401168	13	NULL	NULL	NULL	NULL	Independent variables 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Independent variables were % ibuprofen ( 40 , 60 , 80 ) and % Eudragit RS PO/RL PO ( 0 , 50 , 100 ) .
	manualset3
100340	2	401168	13	NULL	NULL	0	NULL	40 % ibuprofen	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Independent variables were % ibuprofen ( 40 , 60 , 80 ) and % Eudragit RS PO/RL PO ( 0 , 50 , 100 ) .
	manualset3
100341	3	401168	13	NULL	NULL	0	NULL	60 % ibuprofen	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Independent variables were % ibuprofen ( 40 , 60 , 80 ) and % Eudragit RS PO/RL PO ( 0 , 50 , 100 ) .
	manualset3
100344	4	401168	13	NULL	NULL	0	NULL	80 % ibuprofen	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Independent variables were % ibuprofen ( 40 , 60 , 80 ) and % Eudragit RS PO/RL PO ( 0 , 50 , 100 ) .
	manualset3
100346	5	401168	13	NULL	NULL	0	NULL	0% Eudragit RS PO/RL PO	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Independent variables were % ibuprofen ( 40 , 60 , 80 ) and % Eudragit RS PO/RL PO ( 0 , 50 , 100 ) .
	manualset3
100349	6	401168	13	NULL	NULL	0	NULL	50 % Eudragit RS PO/RL PO	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Independent variables were % ibuprofen ( 40 , 60 , 80 ) and % Eudragit RS PO/RL PO ( 0 , 50 , 100 ) .
	manualset3
100350	7	401168	13	NULL	NULL	0	NULL	%100 %Eudragit RS PO/RL PO	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Independent variables were % ibuprofen ( 40 , 60 , 80 ) and % Eudragit RS PO/RL PO ( 0 , 50 , 100 ) .
	manualset3
100351	1	401169	13	NULL	NULL	0	NULL	 left ventricular ( LV ) mass	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Indexed left ventricular ( LV ) mass , LV dimensions , meridional wall stress , and cardiac index were significantly increased .
	manualset3
100352	2	401169	13	NULL	NULL	0	NULL	LV dimensions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Indexed left ventricular ( LV ) mass , LV dimensions , meridional wall stress , and cardiac index were significantly increased .
	manualset3
100353	3	401169	13	NULL	NULL	0	NULL	meridional wall stress 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Indexed left ventricular ( LV ) mass , LV dimensions , meridional wall stress , and cardiac index were significantly increased .
	manualset3
100354	4	401169	13	NULL	NULL	0	NULL	 cardiac index 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Indexed left ventricular ( LV ) mass , LV dimensions , meridional wall stress , and cardiac index were significantly increased .
	manualset3
100355	1	401170	13	NULL	NULL	0	NULL	epitopes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Indicating that only few epitopes are shared by these enzymes , by conventional immuno-diffusion techniques no precipitation lines appeared with antibodies against AK I-HDH I and the other proteins .
	manualset3
100356	2	401170	13	NULL	NULL	0	NULL	enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Indicating that only few epitopes are shared by these enzymes , by conventional immuno-diffusion techniques no precipitation lines appeared with antibodies against AK I-HDH I and the other proteins .
	manualset3
100358	3	401170	13	NULL	NULL	0	NULL	conventional immuno-diffusion techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Indicating that only few epitopes are shared by these enzymes , by conventional immuno-diffusion techniques no precipitation lines appeared with antibodies against AK I-HDH I and the other proteins .
	manualset3
100360	4	401170	13	NULL	NULL	0	NULL	precipitation lines 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Indicating that only few epitopes are shared by these enzymes , by conventional immuno-diffusion techniques no precipitation lines appeared with antibodies against AK I-HDH I and the other proteins .
	manualset3
100361	5	401170	13	NULL	NULL	0	NULL	antibodies 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Indicating that only few epitopes are shared by these enzymes , by conventional immuno-diffusion techniques no precipitation lines appeared with antibodies against AK I-HDH I and the other proteins .
	manualset3
100362	6	401170	13	NULL	NULL	0	NULL	AK I-HDH I 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Indicating that only few epitopes are shared by these enzymes , by conventional immuno-diffusion techniques no precipitation lines appeared with antibodies against AK I-HDH I and the other proteins .
	manualset3
100363	7	401170	13	NULL	NULL	0	NULL	proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Indicating that only few epitopes are shared by these enzymes , by conventional immuno-diffusion techniques no precipitation lines appeared with antibodies against AK I-HDH I and the other proteins .
	manualset3
100365	1	401171	13	NULL	NULL	0	NULL	n the number of vertices of { cal M }	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Indicating with n and s the number of vertices of { cal M } and saddle points of f , the overall computational cost O ( sn ) is competitive with respect to the O ( n , log , n ) cost of previous work .
	manualset3
100366	2	401171	13	NULL	NULL	0	NULL	s the number of saddle points of f	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Indicating with n and s the number of vertices of { cal M } and saddle points of f , the overall computational cost O ( sn ) is competitive with respect to the O ( n , log , n ) cost of previous work .
	manualset3
100367	3	401171	13	NULL	NULL	0	NULL	computational cost O ( sn ) 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Indicating with n and s the number of vertices of { cal M } and saddle points of f , the overall computational cost O ( sn ) is competitive with respect to the O ( n , log , n ) cost of previous work .
	manualset3
100368	4	401171	13	NULL	NULL	0	NULL	respect	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Indicating with n and s the number of vertices of { cal M } and saddle points of f , the overall computational cost O ( sn ) is competitive with respect to the O ( n , log , n ) cost of previous work .
	manualset3
100369	5	401171	13	NULL	NULL	0	NULL	O ( n , log , n ) cost 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Indicating with n and s the number of vertices of { cal M } and saddle points of f , the overall computational cost O ( sn ) is competitive with respect to the O ( n , log , n ) cost of previous work .
	manualset3
100370	6	401171	13	NULL	NULL	0	NULL	work	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Indicating with n and s the number of vertices of { cal M } and saddle points of f , the overall computational cost O ( sn ) is competitive with respect to the O ( n , log , n ) cost of previous work .
	manualset3
100371	1	401172	13	NULL	NULL	NULL	NULL	Indications	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Indications for central vein cannulation or trans-tracheal airway maneuvers must be firm .
	manualset3
100372	2	401172	13	NULL	NULL	0	NULL	central vein cannulation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Indications for central vein cannulation or trans-tracheal airway maneuvers must be firm .
	manualset3
100373	3	401172	13	NULL	NULL	0	NULL	trans-tracheal airway maneuvers	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Indications for central vein cannulation or trans-tracheal airway maneuvers must be firm .
	manualset3
100379	1	401173	13	NULL	NULL	0	NULL	 Indicators	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Indicators of the quality of MOD certification included ( 1 ) MOD not given by the ME/Cs ; ( 2 ) MOD assigned by the ME/Cs was changed by the coder ; ( 3 ) ratio between undetermined and suicide deaths ( U/S ratio ) .
	manualset3
100380	2	401173	13	NULL	NULL	0	NULL	quality of MOD certification	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Indicators of the quality of MOD certification included ( 1 ) MOD not given by the ME/Cs ; ( 2 ) MOD assigned by the ME/Cs was changed by the coder ; ( 3 ) ratio between undetermined and suicide deaths ( U/S ratio ) .
	manualset3
100381	3	401173	13	NULL	NULL	0	NULL	MOD	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Indicators of the quality of MOD certification included ( 1 ) MOD not given by the ME/Cs ; ( 2 ) MOD assigned by the ME/Cs was changed by the coder ; ( 3 ) ratio between undetermined and suicide deaths ( U/S ratio ) .
	manualset3
100383	4	401173	13	NULL	NULL	0	NULL	ME/Cs 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Indicators of the quality of MOD certification included ( 1 ) MOD not given by the ME/Cs ; ( 2 ) MOD assigned by the ME/Cs was changed by the coder ; ( 3 ) ratio between undetermined and suicide deaths ( U/S ratio ) .
	manualset3
100384	5	401173	13	NULL	NULL	0	NULL	MOD	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Indicators of the quality of MOD certification included ( 1 ) MOD not given by the ME/Cs ; ( 2 ) MOD assigned by the ME/Cs was changed by the coder ; ( 3 ) ratio between undetermined and suicide deaths ( U/S ratio ) .
	manualset3
100385	6	401173	13	NULL	NULL	0	NULL	ME/Cs 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Indicators of the quality of MOD certification included ( 1 ) MOD not given by the ME/Cs ; ( 2 ) MOD assigned by the ME/Cs was changed by the coder ; ( 3 ) ratio between undetermined and suicide deaths ( U/S ratio ) .
	manualset3
100386	7	401173	13	NULL	NULL	0	NULL	coder	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Indicators of the quality of MOD certification included ( 1 ) MOD not given by the ME/Cs ; ( 2 ) MOD assigned by the ME/Cs was changed by the coder ; ( 3 ) ratio between undetermined and suicide deaths ( U/S ratio ) .
	manualset3
100387	8	401173	13	NULL	NULL	NULL	NULL	ratio between undetermined and suicide deaths ( U/S ratio ) 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Indicators of the quality of MOD certification included ( 1 ) MOD not given by the ME/Cs ; ( 2 ) MOD assigned by the ME/Cs was changed by the coder ; ( 3 ) ratio between undetermined and suicide deaths ( U/S ratio ) .
	manualset3
100404	1	401174	13	NULL	NULL	0	NULL	Indices	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Indices of expected gain depend directly on the quantity S + T , implying that sensitivity and specificity have equal importance in determining expected gain .
	manualset3
100407	2	401174	13	NULL	NULL	0	NULL	 gain	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Indices of expected gain depend directly on the quantity S + T , implying that sensitivity and specificity have equal importance in determining expected gain .
	manualset3
100409	3	401174	13	NULL	NULL	0	NULL	quantity S + T	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Indices of expected gain depend directly on the quantity S + T , implying that sensitivity and specificity have equal importance in determining expected gain .
	manualset3
100410	4	401174	13	NULL	NULL	0	NULL	sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Indices of expected gain depend directly on the quantity S + T , implying that sensitivity and specificity have equal importance in determining expected gain .
	manualset3
100411	5	401174	13	NULL	NULL	0	NULL	specificity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Indices of expected gain depend directly on the quantity S + T , implying that sensitivity and specificity have equal importance in determining expected gain .
	manualset3
100413	6	401174	13	NULL	NULL	0	NULL	importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Indices of expected gain depend directly on the quantity S + T , implying that sensitivity and specificity have equal importance in determining expected gain .
	manualset3
100414	7	401174	13	NULL	NULL	0	NULL	gain	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Indices of expected gain depend directly on the quantity S + T , implying that sensitivity and specificity have equal importance in determining expected gain .
	manualset3
100417	1	401175	13	NULL	NULL	0	NULL	Indirect binding assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Indirect binding assays utilizing substrate protection against ( 14C ) - N-ethylmaleimide labeling of single-Cys148 permease reveal an apparent Kd of 3-5 mM for lactose and 15-20 microM for beta , D-galactopyranosyl-1-thio-beta , D-galactopyranoside ( TDG ) .
	manualset3
100418	2	401175	13	NULL	NULL	0	NULL	substrate protection against ( 14C ) - N-ethylmaleimide labeling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Indirect binding assays utilizing substrate protection against ( 14C ) - N-ethylmaleimide labeling of single-Cys148 permease reveal an apparent Kd of 3-5 mM for lactose and 15-20 microM for beta , D-galactopyranosyl-1-thio-beta , D-galactopyranoside ( TDG ) .
	manualset3
100421	3	401175	13	NULL	NULL	0	NULL	single-Cys148 permease	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Indirect binding assays utilizing substrate protection against ( 14C ) - N-ethylmaleimide labeling of single-Cys148 permease reveal an apparent Kd of 3-5 mM for lactose and 15-20 microM for beta , D-galactopyranosyl-1-thio-beta , D-galactopyranoside ( TDG ) .
	manualset3
100422	4	401175	13	NULL	NULL	0	NULL	apparent Kd of 3-5 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Indirect binding assays utilizing substrate protection against ( 14C ) - N-ethylmaleimide labeling of single-Cys148 permease reveal an apparent Kd of 3-5 mM for lactose and 15-20 microM for beta , D-galactopyranosyl-1-thio-beta , D-galactopyranoside ( TDG ) .
	manualset3
100423	5	401175	13	NULL	NULL	0	NULL	lactose 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Indirect binding assays utilizing substrate protection against ( 14C ) - N-ethylmaleimide labeling of single-Cys148 permease reveal an apparent Kd of 3-5 mM for lactose and 15-20 microM for beta , D-galactopyranosyl-1-thio-beta , D-galactopyranoside ( TDG ) .
	manualset3
100424	6	401175	13	NULL	NULL	0	NULL	 15-20 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Indirect binding assays utilizing substrate protection against ( 14C ) - N-ethylmaleimide labeling of single-Cys148 permease reveal an apparent Kd of 3-5 mM for lactose and 15-20 microM for beta , D-galactopyranosyl-1-thio-beta , D-galactopyranoside ( TDG ) .
	manualset3
100425	7	401175	13	NULL	NULL	0	NULL	beta , D-galactopyranosyl-1-thio-beta , D-galactopyranoside ( TDG )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Indirect binding assays utilizing substrate protection against ( 14C ) - N-ethylmaleimide labeling of single-Cys148 permease reveal an apparent Kd of 3-5 mM for lactose and 15-20 microM for beta , D-galactopyranosyl-1-thio-beta , D-galactopyranoside ( TDG ) .
	manualset3
100426	1	401176	13	NULL	NULL	0	NULL	Indirect haemagglutination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Indirect haemagglutination and indirect immunofluorescence tests of sera from 95 patients with acute salpingitis failed to confirm the report of other investigators regarding serological evidence implicating Mycoplasma genitalium in pelvic inflammatory disease .
	manualset3
100429	2	401176	13	NULL	NULL	0	NULL	indirect immunofluorescence tests	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Indirect haemagglutination and indirect immunofluorescence tests of sera from 95 patients with acute salpingitis failed to confirm the report of other investigators regarding serological evidence implicating Mycoplasma genitalium in pelvic inflammatory disease .
	manualset3
100430	3	401176	13	NULL	NULL	0	NULL	sera	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Indirect haemagglutination and indirect immunofluorescence tests of sera from 95 patients with acute salpingitis failed to confirm the report of other investigators regarding serological evidence implicating Mycoplasma genitalium in pelvic inflammatory disease .
	manualset3
100432	4	401176	13	NULL	NULL	0	NULL	95 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Indirect haemagglutination and indirect immunofluorescence tests of sera from 95 patients with acute salpingitis failed to confirm the report of other investigators regarding serological evidence implicating Mycoplasma genitalium in pelvic inflammatory disease .
	manualset3
100434	5	401176	13	NULL	NULL	0	NULL	acute salpingitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Indirect haemagglutination and indirect immunofluorescence tests of sera from 95 patients with acute salpingitis failed to confirm the report of other investigators regarding serological evidence implicating Mycoplasma genitalium in pelvic inflammatory disease .
	manualset3
100437	6	401176	13	NULL	NULL	0	NULL	report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Indirect haemagglutination and indirect immunofluorescence tests of sera from 95 patients with acute salpingitis failed to confirm the report of other investigators regarding serological evidence implicating Mycoplasma genitalium in pelvic inflammatory disease .
	manualset3
100438	7	401176	13	NULL	NULL	0	NULL	 investigators	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Indirect haemagglutination and indirect immunofluorescence tests of sera from 95 patients with acute salpingitis failed to confirm the report of other investigators regarding serological evidence implicating Mycoplasma genitalium in pelvic inflammatory disease .
	manualset3
100442	8	401176	13	NULL	NULL	0	NULL	serological evidence 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Indirect haemagglutination and indirect immunofluorescence tests of sera from 95 patients with acute salpingitis failed to confirm the report of other investigators regarding serological evidence implicating Mycoplasma genitalium in pelvic inflammatory disease .
	manualset3
100445	9	401176	13	NULL	NULL	0	NULL	Mycoplasma genitalium	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Indirect haemagglutination and indirect immunofluorescence tests of sera from 95 patients with acute salpingitis failed to confirm the report of other investigators regarding serological evidence implicating Mycoplasma genitalium in pelvic inflammatory disease .
	manualset3
100446	10	401176	13	NULL	NULL	0	NULL	pelvic inflammatory disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Indirect haemagglutination and indirect immunofluorescence tests of sera from 95 patients with acute salpingitis failed to confirm the report of other investigators regarding serological evidence implicating Mycoplasma genitalium in pelvic inflammatory disease .
	manualset3
100453	1	401177	13	NULL	NULL	NULL	NULL	Individual cases	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Individual cases showed a consistent p53 status regardless of the MWH treatment , storage duration , or age of the blocks .
	manualset3
100455	2	401177	13	NULL	NULL	0	NULL	 p53 status	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Individual cases showed a consistent p53 status regardless of the MWH treatment , storage duration , or age of the blocks .
	manualset3
100457	3	401177	13	NULL	NULL	0	NULL	MWH treatment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Individual cases showed a consistent p53 status regardless of the MWH treatment , storage duration , or age of the blocks .
	manualset3
100458	4	401177	13	NULL	NULL	0	NULL	storage duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Individual cases showed a consistent p53 status regardless of the MWH treatment , storage duration , or age of the blocks .
	manualset3
100460	5	401177	13	NULL	NULL	0	NULL	age of the blocks	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Individual cases showed a consistent p53 status regardless of the MWH treatment , storage duration , or age of the blocks .
	manualset3
100466	1	401178	13	NULL	NULL	0	NULL	2003	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	2003 , 11 , 1983-1984 ) except ( Mmt ( 1 ) ) EM-2 ( 7 ) .
	manualset3
100468	2	401178	13	NULL	NULL	0	NULL	11	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2003 , 11 , 1983-1984 ) except ( Mmt ( 1 ) ) EM-2 ( 7 ) .
	manualset3
100470	3	401178	13	NULL	NULL	0	NULL	1983-1984 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2003 , 11 , 1983-1984 ) except ( Mmt ( 1 ) ) EM-2 ( 7 ) .
	manualset3
100473	4	401178	13	NULL	NULL	0	NULL	Mmt ( 1 ) 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	2003 , 11 , 1983-1984 ) except ( Mmt ( 1 ) ) EM-2 ( 7 ) .
	manualset3
100474	5	401178	13	NULL	NULL	0	NULL	EM-2	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	2003 , 11 , 1983-1984 ) except ( Mmt ( 1 ) ) EM-2 ( 7 ) .
	manualset3
100476	1	401179	13	NULL	NULL	0	NULL	Individual molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Individual molecules appear as knotted strands resembling a pretzel ( a pastry snack folded in a unique figure-of-eight ) , which contrasts with our conventional image of collagen molecules as semi-rigid rods .
	manualset3
100482	2	401179	13	NULL	NULL	0	NULL	knotted strands 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Individual molecules appear as knotted strands resembling a pretzel ( a pastry snack folded in a unique figure-of-eight ) , which contrasts with our conventional image of collagen molecules as semi-rigid rods .
	manualset3
100484	3	401179	13	NULL	NULL	0	NULL	pretzel ( a pastry snack folded in a unique figure-of-eight )	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Individual molecules appear as knotted strands resembling a pretzel ( a pastry snack folded in a unique figure-of-eight ) , which contrasts with our conventional image of collagen molecules as semi-rigid rods .
	manualset3
100485	4	401179	13	NULL	NULL	0	NULL	conventional image	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Individual molecules appear as knotted strands resembling a pretzel ( a pastry snack folded in a unique figure-of-eight ) , which contrasts with our conventional image of collagen molecules as semi-rigid rods .
	manualset3
100486	5	401179	13	NULL	NULL	0	NULL	collagen molecules 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Individual molecules appear as knotted strands resembling a pretzel ( a pastry snack folded in a unique figure-of-eight ) , which contrasts with our conventional image of collagen molecules as semi-rigid rods .
	manualset3
100487	6	401179	13	NULL	NULL	0	NULL	semi-rigid rods	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Individual molecules appear as knotted strands resembling a pretzel ( a pastry snack folded in a unique figure-of-eight ) , which contrasts with our conventional image of collagen molecules as semi-rigid rods .
	manualset3
100491	1	401180	13	NULL	NULL	0	NULL	 effects of nisin	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Individual or combined effects of nisin ( 100 or 200 IU/ml ) and the lactoperoxidase system ( LPS ) were analyzed against 1 x 10 ( 4 ) cfu/ml Listeria monocytogenes ATCC 15313 cells in skim milk , at 25 degrees C for 15 days .
	manualset3
100492	2	401180	13	NULL	NULL	0	NULL	100 or 200 IU/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Individual or combined effects of nisin ( 100 or 200 IU/ml ) and the lactoperoxidase system ( LPS ) were analyzed against 1 x 10 ( 4 ) cfu/ml Listeria monocytogenes ATCC 15313 cells in skim milk , at 25 degrees C for 15 days .
	manualset3
100493	3	401180	13	NULL	NULL	0	NULL	effects of lactoperoxidase system ( LPS ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Individual or combined effects of nisin ( 100 or 200 IU/ml ) and the lactoperoxidase system ( LPS ) were analyzed against 1 x 10 ( 4 ) cfu/ml Listeria monocytogenes ATCC 15313 cells in skim milk , at 25 degrees C for 15 days .
	manualset3
100494	4	401180	13	NULL	NULL	NULL	NULL	Listeria monocytogenes ATCC 15313 cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Individual or combined effects of nisin ( 100 or 200 IU/ml ) and the lactoperoxidase system ( LPS ) were analyzed against 1 x 10 ( 4 ) cfu/ml Listeria monocytogenes ATCC 15313 cells in skim milk , at 25 degrees C for 15 days .
	manualset3
100495	5	401180	13	NULL	NULL	0	NULL	skim milk	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Individual or combined effects of nisin ( 100 or 200 IU/ml ) and the lactoperoxidase system ( LPS ) were analyzed against 1 x 10 ( 4 ) cfu/ml Listeria monocytogenes ATCC 15313 cells in skim milk , at 25 degrees C for 15 days .
	manualset3
100496	6	401180	13	NULL	NULL	0	NULL	at 25 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Individual or combined effects of nisin ( 100 or 200 IU/ml ) and the lactoperoxidase system ( LPS ) were analyzed against 1 x 10 ( 4 ) cfu/ml Listeria monocytogenes ATCC 15313 cells in skim milk , at 25 degrees C for 15 days .
	manualset3
100497	7	401180	13	NULL	NULL	0	NULL	15 days	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Individual or combined effects of nisin ( 100 or 200 IU/ml ) and the lactoperoxidase system ( LPS ) were analyzed against 1 x 10 ( 4 ) cfu/ml Listeria monocytogenes ATCC 15313 cells in skim milk , at 25 degrees C for 15 days .
	manualset3
100498	1	401181	13	NULL	NULL	0	NULL	Individual predisposition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Individual predisposition to stress is conceptualized as a latent construct , cognitive-affective stress propensity , that is manifested as multiple trait indicators , e.g. , negative affectivity , anger-irritability , and negative self-esteem .
	manualset3
100499	2	401181	13	NULL	NULL	0	NULL	stress propensity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Individual predisposition to stress is conceptualized as a latent construct , cognitive-affective stress propensity , that is manifested as multiple trait indicators , e.g. , negative affectivity , anger-irritability , and negative self-esteem .
	manualset3
100500	3	401181	13	NULL	NULL	0	NULL	multiple trait indicators	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Individual predisposition to stress is conceptualized as a latent construct , cognitive-affective stress propensity , that is manifested as multiple trait indicators , e.g. , negative affectivity , anger-irritability , and negative self-esteem .
	manualset3
100501	4	401181	13	NULL	NULL	0	NULL	negative affectivity	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Individual predisposition to stress is conceptualized as a latent construct , cognitive-affective stress propensity , that is manifested as multiple trait indicators , e.g. , negative affectivity , anger-irritability , and negative self-esteem .
	manualset3
100502	5	401181	13	NULL	NULL	0	NULL	anger-irritability	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Individual predisposition to stress is conceptualized as a latent construct , cognitive-affective stress propensity , that is manifested as multiple trait indicators , e.g. , negative affectivity , anger-irritability , and negative self-esteem .
	manualset3
100503	6	401181	13	NULL	NULL	0	NULL	 negative self-esteem	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Individual predisposition to stress is conceptualized as a latent construct , cognitive-affective stress propensity , that is manifested as multiple trait indicators , e.g. , negative affectivity , anger-irritability , and negative self-esteem .
	manualset3
100504	1	401182	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Individually tailored treatment with epirubicin and paclitaxel with or without capecitabine as first-line chemotherapy in metastatic breast cancer : a randomized multicenter trial .
	manualset3
100505	2	401182	13	NULL	NULL	0	NULL	 epirubicin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Individually tailored treatment with epirubicin and paclitaxel with or without capecitabine as first-line chemotherapy in metastatic breast cancer : a randomized multicenter trial .
	manualset3
100506	3	401182	13	NULL	NULL	0	NULL	paclitaxel	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Individually tailored treatment with epirubicin and paclitaxel with or without capecitabine as first-line chemotherapy in metastatic breast cancer : a randomized multicenter trial .
	manualset3
100507	4	401182	13	NULL	NULL	0	NULL	capecitabine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Individually tailored treatment with epirubicin and paclitaxel with or without capecitabine as first-line chemotherapy in metastatic breast cancer : a randomized multicenter trial .
	manualset3
100508	5	401182	13	NULL	NULL	0	NULL	first-line chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Individually tailored treatment with epirubicin and paclitaxel with or without capecitabine as first-line chemotherapy in metastatic breast cancer : a randomized multicenter trial .
	manualset3
100509	6	401182	13	NULL	NULL	0	NULL	metastatic breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Individually tailored treatment with epirubicin and paclitaxel with or without capecitabine as first-line chemotherapy in metastatic breast cancer : a randomized multicenter trial .
	manualset3
100511	7	401182	13	NULL	NULL	0	NULL	multicenter trial	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Individually tailored treatment with epirubicin and paclitaxel with or without capecitabine as first-line chemotherapy in metastatic breast cancer : a randomized multicenter trial .
	manualset3
100530	1	401183	13	NULL	NULL	0	NULL	Individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Individuals in the foreclosed identity status group had significantly lower relationship avoidance scores than the diffused identity status group , and the foreclosed group had significantly lower relationship anxiety scores than both the achieved identity and moratorium groups .
	manualset3
100531	2	401183	13	NULL	NULL	NULL	NULL	identity status group	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Individuals in the foreclosed identity status group had significantly lower relationship avoidance scores than the diffused identity status group , and the foreclosed group had significantly lower relationship anxiety scores than both the achieved identity and moratorium groups .
	manualset3
100532	3	401183	13	NULL	NULL	NULL	NULL	relationship avoidance scores	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Individuals in the foreclosed identity status group had significantly lower relationship avoidance scores than the diffused identity status group , and the foreclosed group had significantly lower relationship anxiety scores than both the achieved identity and moratorium groups .
	manualset3
100533	4	401183	13	NULL	NULL	0	NULL	group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Individuals in the foreclosed identity status group had significantly lower relationship avoidance scores than the diffused identity status group , and the foreclosed group had significantly lower relationship anxiety scores than both the achieved identity and moratorium groups .
	manualset3
100534	5	401183	13	NULL	NULL	0	NULL	relationship anxiety scores 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Individuals in the foreclosed identity status group had significantly lower relationship avoidance scores than the diffused identity status group , and the foreclosed group had significantly lower relationship anxiety scores than both the achieved identity and moratorium groups .
	manualset3
100535	6	401183	13	NULL	NULL	0	NULL	identity groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Individuals in the foreclosed identity status group had significantly lower relationship avoidance scores than the diffused identity status group , and the foreclosed group had significantly lower relationship anxiety scores than both the achieved identity and moratorium groups .
	manualset3
100536	7	401183	13	NULL	NULL	0	NULL	moratorium groups 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Individuals in the foreclosed identity status group had significantly lower relationship avoidance scores than the diffused identity status group , and the foreclosed group had significantly lower relationship anxiety scores than both the achieved identity and moratorium groups .
	manualset3
100537	1	401184	13	NULL	NULL	0	NULL	Individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Individuals repeatedly infected with malaria acquire protection from infection and disease ; immunity is thought to be primarily antibody-mediated and directed to blood-stage infection .
	manualset3
100538	2	401184	13	NULL	NULL	0	NULL	malaria 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Individuals repeatedly infected with malaria acquire protection from infection and disease ; immunity is thought to be primarily antibody-mediated and directed to blood-stage infection .
	manualset3
100539	3	401184	13	NULL	NULL	0	NULL	protection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Individuals repeatedly infected with malaria acquire protection from infection and disease ; immunity is thought to be primarily antibody-mediated and directed to blood-stage infection .
	manualset3
100540	4	401184	13	NULL	NULL	0	NULL	infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Individuals repeatedly infected with malaria acquire protection from infection and disease ; immunity is thought to be primarily antibody-mediated and directed to blood-stage infection .
	manualset3
100541	5	401184	13	NULL	NULL	0	NULL	disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Individuals repeatedly infected with malaria acquire protection from infection and disease ; immunity is thought to be primarily antibody-mediated and directed to blood-stage infection .
	manualset3
100542	6	401184	13	NULL	NULL	0	NULL	immunity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Individuals repeatedly infected with malaria acquire protection from infection and disease ; immunity is thought to be primarily antibody-mediated and directed to blood-stage infection .
	manualset3
100543	7	401184	13	NULL	NULL	0	NULL	blood-stage infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Individuals repeatedly infected with malaria acquire protection from infection and disease ; immunity is thought to be primarily antibody-mediated and directed to blood-stage infection .
	manualset3
100544	1	401185	13	NULL	NULL	0	NULL	Individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Individuals with mental health problems may face barriers to accessing effective psychotherapies .
	manualset3
100545	2	401185	13	NULL	NULL	0	NULL	mental health problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Individuals with mental health problems may face barriers to accessing effective psychotherapies .
	manualset3
100546	3	401185	13	NULL	NULL	0	NULL	barriers	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Individuals with mental health problems may face barriers to accessing effective psychotherapies .
	manualset3
100547	4	401185	13	NULL	NULL	0	NULL	effective psychotherapies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Individuals with mental health problems may face barriers to accessing effective psychotherapies .
	manualset3
100548	1	401186	13	NULL	NULL	0	NULL	2009	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	2009 pandemic influenza A ( H1N1 ) virus infections - Chicago , Illinois , April-July 2009 .
	manualset3
100549	2	401186	13	NULL	NULL	0	NULL	 pandemic influenza A ( H1N1 ) virus infections 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	2009 pandemic influenza A ( H1N1 ) virus infections - Chicago , Illinois , April-July 2009 .
	manualset3
100550	3	401186	13	NULL	NULL	0	NULL	Chicago	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	2009 pandemic influenza A ( H1N1 ) virus infections - Chicago , Illinois , April-July 2009 .
	manualset3
100551	4	401186	13	NULL	NULL	0	NULL	Illinois 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	2009 pandemic influenza A ( H1N1 ) virus infections - Chicago , Illinois , April-July 2009 .
	manualset3
100552	5	401186	13	NULL	NULL	0	NULL	April-July 2009 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	2009 pandemic influenza A ( H1N1 ) virus infections - Chicago , Illinois , April-July 2009 .
	manualset3
100553	1	401187	13	NULL	NULL	0	NULL	Indomethacin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Indomethacin , a COX inhibitor , at 5 mg/kg , but not 10 mg/kg , suppressed significantly the LPS-induced increase in the brain fluorescein level .
	manualset3
100554	2	401187	13	NULL	NULL	0	NULL	COX inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Indomethacin , a COX inhibitor , at 5 mg/kg , but not 10 mg/kg , suppressed significantly the LPS-induced increase in the brain fluorescein level .
	manualset3
100555	3	401187	13	NULL	NULL	0	NULL	5 mg/kg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Indomethacin , a COX inhibitor , at 5 mg/kg , but not 10 mg/kg , suppressed significantly the LPS-induced increase in the brain fluorescein level .
	manualset3
100556	4	401187	13	NULL	NULL	0	NULL	10 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Indomethacin , a COX inhibitor , at 5 mg/kg , but not 10 mg/kg , suppressed significantly the LPS-induced increase in the brain fluorescein level .
	manualset3
100557	5	401187	13	NULL	NULL	0	NULL	LPS-induced increase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Indomethacin , a COX inhibitor , at 5 mg/kg , but not 10 mg/kg , suppressed significantly the LPS-induced increase in the brain fluorescein level .
	manualset3
100558	6	401187	13	NULL	NULL	0	NULL	brain fluorescein level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Indomethacin , a COX inhibitor , at 5 mg/kg , but not 10 mg/kg , suppressed significantly the LPS-induced increase in the brain fluorescein level .
	manualset3
100559	1	401188	13	NULL	NULL	0	NULL	Indomethacin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Indomethacin and VIP-antiserum inhibited the Ca2 + , HCO ( 3 ) - and fluid secretion across the inflamed gallbladder mucosa .
	manualset3
100563	2	401188	13	NULL	NULL	0	NULL	VIP-antiserum 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Indomethacin and VIP-antiserum inhibited the Ca2 + , HCO ( 3 ) - and fluid secretion across the inflamed gallbladder mucosa .
	manualset3
100565	3	401188	13	NULL	NULL	0	NULL	Ca2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Indomethacin and VIP-antiserum inhibited the Ca2 + , HCO ( 3 ) - and fluid secretion across the inflamed gallbladder mucosa .
	manualset3
100566	4	401188	13	NULL	NULL	0	NULL	HCO ( 3 ) -	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Indomethacin and VIP-antiserum inhibited the Ca2 + , HCO ( 3 ) - and fluid secretion across the inflamed gallbladder mucosa .
	manualset3
100567	5	401188	13	NULL	NULL	0	NULL	fluid secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Indomethacin and VIP-antiserum inhibited the Ca2 + , HCO ( 3 ) - and fluid secretion across the inflamed gallbladder mucosa .
	manualset3
100568	6	401188	13	NULL	NULL	0	NULL	inflamed gallbladder mucosa 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Indomethacin and VIP-antiserum inhibited the Ca2 + , HCO ( 3 ) - and fluid secretion across the inflamed gallbladder mucosa .
	manualset3
100572	1	401189	13	NULL	NULL	0	NULL	tolerance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Induced tolerance , cross resistance .
	manualset3
100574	2	401189	13	NULL	NULL	0	NULL	resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Induced tolerance , cross resistance .
	manualset3
100575	1	401190	13	NULL	NULL	0	NULL	 tyrosine phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Induced tyrosine phosphorylation of several proteins was seen after ephrin-A1 binding .
	manualset3
100576	2	401190	13	NULL	NULL	0	NULL	several proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Induced tyrosine phosphorylation of several proteins was seen after ephrin-A1 binding .
	manualset3
100577	3	401190	13	NULL	NULL	0	NULL	ephrin-A1 binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Induced tyrosine phosphorylation of several proteins was seen after ephrin-A1 binding .
	manualset3
100580	1	401191	13	NULL	NULL	0	NULL	Induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of LOX-1 gene expression by high glucose was abolished by antioxidants , protein kinase C ( PKC ) , mitogen-activated protein kinases ( MAPKs ) , nuclear factor-kappaB ( NF-kappaB ) , and activated protein-1 ( AP-1 ) inhibitors .
	manualset3
100582	2	401191	13	NULL	NULL	0	NULL	LOX-1 gene expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of LOX-1 gene expression by high glucose was abolished by antioxidants , protein kinase C ( PKC ) , mitogen-activated protein kinases ( MAPKs ) , nuclear factor-kappaB ( NF-kappaB ) , and activated protein-1 ( AP-1 ) inhibitors .
	manualset3
100583	3	401191	13	NULL	NULL	0	NULL	glucose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of LOX-1 gene expression by high glucose was abolished by antioxidants , protein kinase C ( PKC ) , mitogen-activated protein kinases ( MAPKs ) , nuclear factor-kappaB ( NF-kappaB ) , and activated protein-1 ( AP-1 ) inhibitors .
	manualset3
100584	4	401191	13	NULL	NULL	0	NULL	antioxidants	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of LOX-1 gene expression by high glucose was abolished by antioxidants , protein kinase C ( PKC ) , mitogen-activated protein kinases ( MAPKs ) , nuclear factor-kappaB ( NF-kappaB ) , and activated protein-1 ( AP-1 ) inhibitors .
	manualset3
100585	5	401191	13	NULL	NULL	NULL	NULL	protein kinase C ( PKC ) inhibitors	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Induction of LOX-1 gene expression by high glucose was abolished by antioxidants , protein kinase C ( PKC ) , mitogen-activated protein kinases ( MAPKs ) , nuclear factor-kappaB ( NF-kappaB ) , and activated protein-1 ( AP-1 ) inhibitors .
	manualset3
100587	6	401191	13	NULL	NULL	NULL	NULL	mitogen-activated protein kinases ( MAPKs ) inhibitors	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Induction of LOX-1 gene expression by high glucose was abolished by antioxidants , protein kinase C ( PKC ) , mitogen-activated protein kinases ( MAPKs ) , nuclear factor-kappaB ( NF-kappaB ) , and activated protein-1 ( AP-1 ) inhibitors .
	manualset3
100588	7	401191	13	NULL	NULL	0	NULL	nuclear factor-kappaB ( NF-kappaB ) inhibitors 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of LOX-1 gene expression by high glucose was abolished by antioxidants , protein kinase C ( PKC ) , mitogen-activated protein kinases ( MAPKs ) , nuclear factor-kappaB ( NF-kappaB ) , and activated protein-1 ( AP-1 ) inhibitors .
	manualset3
100589	8	401191	13	NULL	NULL	0	NULL	activated protein-1 ( AP-1 ) inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of LOX-1 gene expression by high glucose was abolished by antioxidants , protein kinase C ( PKC ) , mitogen-activated protein kinases ( MAPKs ) , nuclear factor-kappaB ( NF-kappaB ) , and activated protein-1 ( AP-1 ) inhibitors .
	manualset3
100590	1	401192	13	NULL	NULL	0	NULL	Induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of PGHS-2 RNA in IFN-gamma-treated NHBECs , which peaked at 24 h , suggested the presence of an intermediary substance regulating the expression of PGHS-2 .
	manualset3
100591	2	401192	13	NULL	NULL	0	NULL	PGHS-2 RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of PGHS-2 RNA in IFN-gamma-treated NHBECs , which peaked at 24 h , suggested the presence of an intermediary substance regulating the expression of PGHS-2 .
	manualset3
100592	3	401192	13	NULL	NULL	0	NULL	 IFN-gamma-treated NHBECs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of PGHS-2 RNA in IFN-gamma-treated NHBECs , which peaked at 24 h , suggested the presence of an intermediary substance regulating the expression of PGHS-2 .
	manualset3
100593	4	401192	13	NULL	NULL	0	NULL	24 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of PGHS-2 RNA in IFN-gamma-treated NHBECs , which peaked at 24 h , suggested the presence of an intermediary substance regulating the expression of PGHS-2 .
	manualset3
100594	5	401192	13	NULL	NULL	NULL	NULL	presence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Induction of PGHS-2 RNA in IFN-gamma-treated NHBECs , which peaked at 24 h , suggested the presence of an intermediary substance regulating the expression of PGHS-2 .
	manualset3
100595	6	401192	13	NULL	NULL	0	NULL	 intermediary substance	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of PGHS-2 RNA in IFN-gamma-treated NHBECs , which peaked at 24 h , suggested the presence of an intermediary substance regulating the expression of PGHS-2 .
	manualset3
100596	7	401192	13	NULL	NULL	0	NULL	expression of PGHS-2	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of PGHS-2 RNA in IFN-gamma-treated NHBECs , which peaked at 24 h , suggested the presence of an intermediary substance regulating the expression of PGHS-2 .
	manualset3
100597	1	401193	13	NULL	NULL	NULL	NULL	Induction	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Induction of antigen-specific human CD4 ( + ) T cell anergy by peripheral blood DC2 precursors .
	manualset3
100598	2	401193	13	NULL	NULL	0	NULL	 human CD4 ( + ) T cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of antigen-specific human CD4 ( + ) T cell anergy by peripheral blood DC2 precursors .
	manualset3
100599	3	401193	13	NULL	NULL	0	NULL	anergy 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of antigen-specific human CD4 ( + ) T cell anergy by peripheral blood DC2 precursors .
	manualset3
100600	4	401193	13	NULL	NULL	0	NULL	peripheral blood DC2 precursors	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of antigen-specific human CD4 ( + ) T cell anergy by peripheral blood DC2 precursors .
	manualset3
100601	1	401194	13	NULL	NULL	0	NULL	Induction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of cell death in human papillomavirus 18-positive cervical cancer cells by E6 siRNA .
	manualset3
100602	2	401194	13	NULL	NULL	0	NULL	cell death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of cell death in human papillomavirus 18-positive cervical cancer cells by E6 siRNA .
	manualset3
100604	3	401194	13	NULL	NULL	0	NULL	human papillomavirus 18-positive cervical cancer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of cell death in human papillomavirus 18-positive cervical cancer cells by E6 siRNA .
	manualset3
100605	4	401194	13	NULL	NULL	0	NULL	E6 siRNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of cell death in human papillomavirus 18-positive cervical cancer cells by E6 siRNA .
	manualset3
100606	1	401195	13	NULL	NULL	0	NULL	Induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of nitric oxide synthase is involved in the mechanism of Fas-mediated apoptosis in hemopoietic cells .
	manualset3
100607	2	401195	13	NULL	NULL	0	NULL	nitric oxide synthase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of nitric oxide synthase is involved in the mechanism of Fas-mediated apoptosis in hemopoietic cells .
	manualset3
100609	3	401195	13	NULL	NULL	0	NULL	 mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of nitric oxide synthase is involved in the mechanism of Fas-mediated apoptosis in hemopoietic cells .
	manualset3
100611	4	401195	13	NULL	NULL	0	NULL	Fas-mediated apoptosis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of nitric oxide synthase is involved in the mechanism of Fas-mediated apoptosis in hemopoietic cells .
	manualset3
100613	5	401195	13	NULL	NULL	0	NULL	hemopoietic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of nitric oxide synthase is involved in the mechanism of Fas-mediated apoptosis in hemopoietic cells .
	manualset3
100616	1	401196	13	NULL	NULL	0	NULL	Association 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	( Association of L-selectin gene polymorphism with susceptibility to coronary heart disease ) .
	manualset3
100617	2	401196	13	NULL	NULL	0	NULL	L-selectin gene polymorphism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Association of L-selectin gene polymorphism with susceptibility to coronary heart disease ) .
	manualset3
100627	3	401196	13	NULL	NULL	0	NULL	susceptibility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Association of L-selectin gene polymorphism with susceptibility to coronary heart disease ) .
	manualset3
100629	4	401196	13	NULL	NULL	0	NULL	coronary heart disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Association of L-selectin gene polymorphism with susceptibility to coronary heart disease ) .
	manualset3
100631	1	401197	13	NULL	NULL	0	NULL	2010	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	2010 European guideline for the management of Chlamydia trachomatis infections .
	manualset3
100632	2	401197	13	NULL	NULL	0	NULL	European guideline	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	2010 European guideline for the management of Chlamydia trachomatis infections .
	manualset3
100633	3	401197	13	NULL	NULL	0	NULL	management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	2010 European guideline for the management of Chlamydia trachomatis infections .
	manualset3
100634	4	401197	13	NULL	NULL	0	NULL	Chlamydia trachomatis infections 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	2010 European guideline for the management of Chlamydia trachomatis infections .
	manualset3
100635	1	401198	13	NULL	NULL	0	NULL	Induction of photolyase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of photolyase was observed in response to greater ambient UV-R ( such as shallower water depths or sea ice-free regions ) .
	manualset3
100636	2	401198	13	NULL	NULL	0	NULL	response	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of photolyase was observed in response to greater ambient UV-R ( such as shallower water depths or sea ice-free regions ) .
	manualset3
100637	3	401198	13	NULL	NULL	0	NULL	ambient UV-R	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of photolyase was observed in response to greater ambient UV-R ( such as shallower water depths or sea ice-free regions ) .
	manualset3
100638	4	401198	13	NULL	NULL	0	NULL	shallower water depths	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of photolyase was observed in response to greater ambient UV-R ( such as shallower water depths or sea ice-free regions ) .
	manualset3
100639	5	401198	13	NULL	NULL	0	NULL	sea ice-free regions	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of photolyase was observed in response to greater ambient UV-R ( such as shallower water depths or sea ice-free regions ) .
	manualset3
100676	1	401199	13	NULL	NULL	0	NULL	Induction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of the CCM , as measured by silicone oil centrifugation , was hindered in the presence of rifampin .
	manualset3
100677	2	401199	13	NULL	NULL	0	NULL	CCM	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of the CCM , as measured by silicone oil centrifugation , was hindered in the presence of rifampin .
	manualset3
100678	3	401199	13	NULL	NULL	0	NULL	silicone oil centrifugation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of the CCM , as measured by silicone oil centrifugation , was hindered in the presence of rifampin .
	manualset3
100679	4	401199	13	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of the CCM , as measured by silicone oil centrifugation , was hindered in the presence of rifampin .
	manualset3
100680	5	401199	13	NULL	NULL	0	NULL	rifampin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of the CCM , as measured by silicone oil centrifugation , was hindered in the presence of rifampin .
	manualset3
100681	1	401200	13	NULL	NULL	0	NULL	Infant pertussis deaths	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infant pertussis deaths and the management of cardiovascular compromise .
	manualset3
100682	2	401200	13	NULL	NULL	0	NULL	management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Infant pertussis deaths and the management of cardiovascular compromise .
	manualset3
100683	3	401200	13	NULL	NULL	0	NULL	cardiovascular compromise	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infant pertussis deaths and the management of cardiovascular compromise .
	manualset3
100684	1	401201	13	NULL	NULL	0	NULL	Infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants familiarized with a melody for 7 days preferred , on the eighth day , to listen to a novel melody in comparison to the familiarized one , regardless of whether the melodies at test were presented at the same pitch as during familiarization or transposed up or down by a perfect fifth ( 7/12th of an octave ) or a tritone ( 1/2 octave ) .
	manualset3
100685	2	401201	13	NULL	NULL	0	NULL	melody	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants familiarized with a melody for 7 days preferred , on the eighth day , to listen to a novel melody in comparison to the familiarized one , regardless of whether the melodies at test were presented at the same pitch as during familiarization or transposed up or down by a perfect fifth ( 7/12th of an octave ) or a tritone ( 1/2 octave ) .
	manualset3
100686	3	401201	13	NULL	NULL	0	NULL	7 days	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants familiarized with a melody for 7 days preferred , on the eighth day , to listen to a novel melody in comparison to the familiarized one , regardless of whether the melodies at test were presented at the same pitch as during familiarization or transposed up or down by a perfect fifth ( 7/12th of an octave ) or a tritone ( 1/2 octave ) .
	manualset3
100687	4	401201	13	NULL	NULL	0	NULL	eighth day	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants familiarized with a melody for 7 days preferred , on the eighth day , to listen to a novel melody in comparison to the familiarized one , regardless of whether the melodies at test were presented at the same pitch as during familiarization or transposed up or down by a perfect fifth ( 7/12th of an octave ) or a tritone ( 1/2 octave ) .
	manualset3
100688	5	401201	13	NULL	NULL	0	NULL	novel melody	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants familiarized with a melody for 7 days preferred , on the eighth day , to listen to a novel melody in comparison to the familiarized one , regardless of whether the melodies at test were presented at the same pitch as during familiarization or transposed up or down by a perfect fifth ( 7/12th of an octave ) or a tritone ( 1/2 octave ) .
	manualset3
100689	6	401201	13	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants familiarized with a melody for 7 days preferred , on the eighth day , to listen to a novel melody in comparison to the familiarized one , regardless of whether the melodies at test were presented at the same pitch as during familiarization or transposed up or down by a perfect fifth ( 7/12th of an octave ) or a tritone ( 1/2 octave ) .
	manualset3
100690	7	401201	13	NULL	NULL	0	NULL	familiarized one	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants familiarized with a melody for 7 days preferred , on the eighth day , to listen to a novel melody in comparison to the familiarized one , regardless of whether the melodies at test were presented at the same pitch as during familiarization or transposed up or down by a perfect fifth ( 7/12th of an octave ) or a tritone ( 1/2 octave ) .
	manualset3
100691	8	401201	13	NULL	NULL	0	NULL	 melodies	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants familiarized with a melody for 7 days preferred , on the eighth day , to listen to a novel melody in comparison to the familiarized one , regardless of whether the melodies at test were presented at the same pitch as during familiarization or transposed up or down by a perfect fifth ( 7/12th of an octave ) or a tritone ( 1/2 octave ) .
	manualset3
100692	9	401201	13	NULL	NULL	0	NULL	test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants familiarized with a melody for 7 days preferred , on the eighth day , to listen to a novel melody in comparison to the familiarized one , regardless of whether the melodies at test were presented at the same pitch as during familiarization or transposed up or down by a perfect fifth ( 7/12th of an octave ) or a tritone ( 1/2 octave ) .
	manualset3
100693	10	401201	13	NULL	NULL	0	NULL	 pitch	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants familiarized with a melody for 7 days preferred , on the eighth day , to listen to a novel melody in comparison to the familiarized one , regardless of whether the melodies at test were presented at the same pitch as during familiarization or transposed up or down by a perfect fifth ( 7/12th of an octave ) or a tritone ( 1/2 octave ) .
	manualset3
100694	11	401201	13	NULL	NULL	0	NULL	familiarization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants familiarized with a melody for 7 days preferred , on the eighth day , to listen to a novel melody in comparison to the familiarized one , regardless of whether the melodies at test were presented at the same pitch as during familiarization or transposed up or down by a perfect fifth ( 7/12th of an octave ) or a tritone ( 1/2 octave ) .
	manualset3
100695	12	401201	13	NULL	NULL	NULL	NULL	perfect fifth ( 7/12th of an octave ) 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Infants familiarized with a melody for 7 days preferred , on the eighth day , to listen to a novel melody in comparison to the familiarized one , regardless of whether the melodies at test were presented at the same pitch as during familiarization or transposed up or down by a perfect fifth ( 7/12th of an octave ) or a tritone ( 1/2 octave ) .
	manualset3
100696	13	401201	13	NULL	NULL	0	NULL	tritone ( 1/2 octave ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants familiarized with a melody for 7 days preferred , on the eighth day , to listen to a novel melody in comparison to the familiarized one , regardless of whether the melodies at test were presented at the same pitch as during familiarization or transposed up or down by a perfect fifth ( 7/12th of an octave ) or a tritone ( 1/2 octave ) .
	manualset3
100697	1	401202	13	NULL	NULL	0	NULL	Infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants hearing music had significantly fewer occurrences of Oximeter alarms during auditory stimuli than did those listening to the mothers ' voice .
	manualset3
100698	2	401202	13	NULL	NULL	0	NULL	hearing music 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants hearing music had significantly fewer occurrences of Oximeter alarms during auditory stimuli than did those listening to the mothers ' voice .
	manualset3
100699	3	401202	13	NULL	NULL	NULL	NULL	occurrences	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Infants hearing music had significantly fewer occurrences of Oximeter alarms during auditory stimuli than did those listening to the mothers ' voice .
	manualset3
100700	4	401202	13	NULL	NULL	0	NULL	Oximeter alarms	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants hearing music had significantly fewer occurrences of Oximeter alarms during auditory stimuli than did those listening to the mothers ' voice .
	manualset3
100701	5	401202	13	NULL	NULL	0	NULL	auditory stimuli 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants hearing music had significantly fewer occurrences of Oximeter alarms during auditory stimuli than did those listening to the mothers ' voice .
	manualset3
100702	6	401202	13	NULL	NULL	NULL	NULL	 mothers 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Infants hearing music had significantly fewer occurrences of Oximeter alarms during auditory stimuli than did those listening to the mothers ' voice .
	manualset3
100703	7	401202	13	NULL	NULL	NULL	NULL	voice	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Infants hearing music had significantly fewer occurrences of Oximeter alarms during auditory stimuli than did those listening to the mothers ' voice .
	manualset3
100704	1	401203	13	NULL	NULL	0	NULL	Infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants with birthweights ) or = 4 , 500 gm were 7.0 times more likely ( 95 % confidence interval = 5.4-9 .1 ) to have a subsequent macrosomic sibling than were infants with smaller birthweights , after controlling for pregnancy smoking status , parity , and gestational age .
	manualset3
100705	2	401203	13	NULL	NULL	0	NULL	birthweights ) or = 4 , 500 gm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants with birthweights ) or = 4 , 500 gm were 7.0 times more likely ( 95 % confidence interval = 5.4-9 .1 ) to have a subsequent macrosomic sibling than were infants with smaller birthweights , after controlling for pregnancy smoking status , parity , and gestational age .
	manualset3
100706	3	401203	13	NULL	NULL	0	NULL	7.0 times 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants with birthweights ) or = 4 , 500 gm were 7.0 times more likely ( 95 % confidence interval = 5.4-9 .1 ) to have a subsequent macrosomic sibling than were infants with smaller birthweights , after controlling for pregnancy smoking status , parity , and gestational age .
	manualset3
100707	4	401203	13	NULL	NULL	0	NULL	95 % confidence interval = 5.4-9 .1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants with birthweights ) or = 4 , 500 gm were 7.0 times more likely ( 95 % confidence interval = 5.4-9 .1 ) to have a subsequent macrosomic sibling than were infants with smaller birthweights , after controlling for pregnancy smoking status , parity , and gestational age .
	manualset3
100708	5	401203	13	NULL	NULL	0	NULL	macrosomic sibling 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants with birthweights ) or = 4 , 500 gm were 7.0 times more likely ( 95 % confidence interval = 5.4-9 .1 ) to have a subsequent macrosomic sibling than were infants with smaller birthweights , after controlling for pregnancy smoking status , parity , and gestational age .
	manualset3
100709	6	401203	13	NULL	NULL	0	NULL	infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants with birthweights ) or = 4 , 500 gm were 7.0 times more likely ( 95 % confidence interval = 5.4-9 .1 ) to have a subsequent macrosomic sibling than were infants with smaller birthweights , after controlling for pregnancy smoking status , parity , and gestational age .
	manualset3
100710	7	401203	13	NULL	NULL	0	NULL	smaller birthweights	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants with birthweights ) or = 4 , 500 gm were 7.0 times more likely ( 95 % confidence interval = 5.4-9 .1 ) to have a subsequent macrosomic sibling than were infants with smaller birthweights , after controlling for pregnancy smoking status , parity , and gestational age .
	manualset3
100711	8	401203	13	NULL	NULL	0	NULL	pregnancy smoking status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants with birthweights ) or = 4 , 500 gm were 7.0 times more likely ( 95 % confidence interval = 5.4-9 .1 ) to have a subsequent macrosomic sibling than were infants with smaller birthweights , after controlling for pregnancy smoking status , parity , and gestational age .
	manualset3
100712	9	401203	13	NULL	NULL	0	NULL	parity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants with birthweights ) or = 4 , 500 gm were 7.0 times more likely ( 95 % confidence interval = 5.4-9 .1 ) to have a subsequent macrosomic sibling than were infants with smaller birthweights , after controlling for pregnancy smoking status , parity , and gestational age .
	manualset3
100713	10	401203	13	NULL	NULL	0	NULL	gestational age 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants with birthweights ) or = 4 , 500 gm were 7.0 times more likely ( 95 % confidence interval = 5.4-9 .1 ) to have a subsequent macrosomic sibling than were infants with smaller birthweights , after controlling for pregnancy smoking status , parity , and gestational age .
	manualset3
100714	1	401204	13	NULL	NULL	0	NULL	 kidneys	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Infected kidneys appeared to be more susceptible to the nephrotoxic potential of gentamicin .
	manualset3
100715	2	401204	13	NULL	NULL	0	NULL	nephrotoxic potential 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infected kidneys appeared to be more susceptible to the nephrotoxic potential of gentamicin .
	manualset3
100716	3	401204	13	NULL	NULL	0	NULL	gentamicin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Infected kidneys appeared to be more susceptible to the nephrotoxic potential of gentamicin .
	manualset3
100717	1	401205	13	NULL	NULL	0	NULL	pancreatic necrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infected pancreatic necrosis is a devastating and lethal complication of acute pancreatitis .
	manualset3
100718	2	401205	13	NULL	NULL	0	NULL	devastating complication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infected pancreatic necrosis is a devastating and lethal complication of acute pancreatitis .
	manualset3
100719	3	401205	13	NULL	NULL	0	NULL	lethal complication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infected pancreatic necrosis is a devastating and lethal complication of acute pancreatitis .
	manualset3
100720	4	401205	13	NULL	NULL	0	NULL	acute pancreatitis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infected pancreatic necrosis is a devastating and lethal complication of acute pancreatitis .
	manualset3
100721	1	401206	13	NULL	NULL	0	NULL	Infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection and autoimmunity : theme and variations .
	manualset3
100722	2	401206	13	NULL	NULL	0	NULL	autoimmunity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection and autoimmunity : theme and variations .
	manualset3
100723	3	401206	13	NULL	NULL	0	NULL	theme	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection and autoimmunity : theme and variations .
	manualset3
100724	4	401206	13	NULL	NULL	0	NULL	variations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection and autoimmunity : theme and variations .
	manualset3
100725	1	401207	13	NULL	NULL	0	NULL	Infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection in the presence of 0.5 M BQR reduced virus progeny production by & gt ; 90 % , revealing an EC ( 50 ) ( drug concentration required to inhibit 50 % of virus replication ) of 0.017 M. Replication of other orthopoxviruses was also inhibited by BQR at similar levels .
	manualset3
100726	2	401207	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection in the presence of 0.5 M BQR reduced virus progeny production by & gt ; 90 % , revealing an EC ( 50 ) ( drug concentration required to inhibit 50 % of virus replication ) of 0.017 M. Replication of other orthopoxviruses was also inhibited by BQR at similar levels .
	manualset3
100727	3	401207	13	NULL	NULL	0	NULL	0.5 M BQR	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection in the presence of 0.5 M BQR reduced virus progeny production by & gt ; 90 % , revealing an EC ( 50 ) ( drug concentration required to inhibit 50 % of virus replication ) of 0.017 M. Replication of other orthopoxviruses was also inhibited by BQR at similar levels .
	manualset3
100728	4	401207	13	NULL	NULL	0	NULL	 virus progeny production 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection in the presence of 0.5 M BQR reduced virus progeny production by & gt ; 90 % , revealing an EC ( 50 ) ( drug concentration required to inhibit 50 % of virus replication ) of 0.017 M. Replication of other orthopoxviruses was also inhibited by BQR at similar levels .
	manualset3
100729	5	401207	13	NULL	NULL	0	NULL	90 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection in the presence of 0.5 M BQR reduced virus progeny production by & gt ; 90 % , revealing an EC ( 50 ) ( drug concentration required to inhibit 50 % of virus replication ) of 0.017 M. Replication of other orthopoxviruses was also inhibited by BQR at similar levels .
	manualset3
100730	6	401207	13	NULL	NULL	0	NULL	EC ( 50 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection in the presence of 0.5 M BQR reduced virus progeny production by & gt ; 90 % , revealing an EC ( 50 ) ( drug concentration required to inhibit 50 % of virus replication ) of 0.017 M. Replication of other orthopoxviruses was also inhibited by BQR at similar levels .
	manualset3
100731	7	401207	13	NULL	NULL	0	NULL	drug concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection in the presence of 0.5 M BQR reduced virus progeny production by & gt ; 90 % , revealing an EC ( 50 ) ( drug concentration required to inhibit 50 % of virus replication ) of 0.017 M. Replication of other orthopoxviruses was also inhibited by BQR at similar levels .
	manualset3
100732	8	401207	13	NULL	NULL	0	NULL	50 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection in the presence of 0.5 M BQR reduced virus progeny production by & gt ; 90 % , revealing an EC ( 50 ) ( drug concentration required to inhibit 50 % of virus replication ) of 0.017 M. Replication of other orthopoxviruses was also inhibited by BQR at similar levels .
	manualset3
100733	9	401207	13	NULL	NULL	0	NULL	virus replication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection in the presence of 0.5 M BQR reduced virus progeny production by & gt ; 90 % , revealing an EC ( 50 ) ( drug concentration required to inhibit 50 % of virus replication ) of 0.017 M. Replication of other orthopoxviruses was also inhibited by BQR at similar levels .
	manualset3
100734	10	401207	13	NULL	NULL	0	NULL	0.017 M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection in the presence of 0.5 M BQR reduced virus progeny production by & gt ; 90 % , revealing an EC ( 50 ) ( drug concentration required to inhibit 50 % of virus replication ) of 0.017 M. Replication of other orthopoxviruses was also inhibited by BQR at similar levels .
	manualset3
100735	11	401207	13	NULL	NULL	0	NULL	Replication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection in the presence of 0.5 M BQR reduced virus progeny production by & gt ; 90 % , revealing an EC ( 50 ) ( drug concentration required to inhibit 50 % of virus replication ) of 0.017 M. Replication of other orthopoxviruses was also inhibited by BQR at similar levels .
	manualset3
100736	12	401207	13	NULL	NULL	0	NULL	orthopoxviruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection in the presence of 0.5 M BQR reduced virus progeny production by & gt ; 90 % , revealing an EC ( 50 ) ( drug concentration required to inhibit 50 % of virus replication ) of 0.017 M. Replication of other orthopoxviruses was also inhibited by BQR at similar levels .
	manualset3
100737	13	401207	13	NULL	NULL	0	NULL	BQR 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection in the presence of 0.5 M BQR reduced virus progeny production by & gt ; 90 % , revealing an EC ( 50 ) ( drug concentration required to inhibit 50 % of virus replication ) of 0.017 M. Replication of other orthopoxviruses was also inhibited by BQR at similar levels .
	manualset3
100738	14	401207	13	NULL	NULL	0	NULL	levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection in the presence of 0.5 M BQR reduced virus progeny production by & gt ; 90 % , revealing an EC ( 50 ) ( drug concentration required to inhibit 50 % of virus replication ) of 0.017 M. Replication of other orthopoxviruses was also inhibited by BQR at similar levels .
	manualset3
100739	1	401208	13	NULL	NULL	0	NULL	Infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection significantly increased ( P & lt ; 0.05 ) the contribution of transsulfuration to cysteine flux in both plasma and liver ( by 80 % ) and the contribution of transsulfuration to plasma methionine flux ( by 133 % ) .
	manualset3
100740	2	401208	13	NULL	NULL	0	NULL	P & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection significantly increased ( P & lt ; 0.05 ) the contribution of transsulfuration to cysteine flux in both plasma and liver ( by 80 % ) and the contribution of transsulfuration to plasma methionine flux ( by 133 % ) .
	manualset3
100741	3	401208	13	NULL	NULL	0	NULL	contribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection significantly increased ( P & lt ; 0.05 ) the contribution of transsulfuration to cysteine flux in both plasma and liver ( by 80 % ) and the contribution of transsulfuration to plasma methionine flux ( by 133 % ) .
	manualset3
100742	4	401208	13	NULL	NULL	NULL	NULL	transsulfuration	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Infection significantly increased ( P & lt ; 0.05 ) the contribution of transsulfuration to cysteine flux in both plasma and liver ( by 80 % ) and the contribution of transsulfuration to plasma methionine flux ( by 133 % ) .
	manualset3
100743	5	401208	13	NULL	NULL	NULL	NULL	cysteine flux 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Infection significantly increased ( P & lt ; 0.05 ) the contribution of transsulfuration to cysteine flux in both plasma and liver ( by 80 % ) and the contribution of transsulfuration to plasma methionine flux ( by 133 % ) .
	manualset3
100744	6	401208	13	NULL	NULL	0	NULL	plasma	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection significantly increased ( P & lt ; 0.05 ) the contribution of transsulfuration to cysteine flux in both plasma and liver ( by 80 % ) and the contribution of transsulfuration to plasma methionine flux ( by 133 % ) .
	manualset3
100745	7	401208	13	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection significantly increased ( P & lt ; 0.05 ) the contribution of transsulfuration to cysteine flux in both plasma and liver ( by 80 % ) and the contribution of transsulfuration to plasma methionine flux ( by 133 % ) .
	manualset3
100746	8	401208	13	NULL	NULL	0	NULL	by 80 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection significantly increased ( P & lt ; 0.05 ) the contribution of transsulfuration to cysteine flux in both plasma and liver ( by 80 % ) and the contribution of transsulfuration to plasma methionine flux ( by 133 % ) .
	manualset3
100747	9	401208	13	NULL	NULL	0	NULL	transsulfuration	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection significantly increased ( P & lt ; 0.05 ) the contribution of transsulfuration to cysteine flux in both plasma and liver ( by 80 % ) and the contribution of transsulfuration to plasma methionine flux ( by 133 % ) .
	manualset3
100748	10	401208	13	NULL	NULL	0	NULL	plasma methionine flux 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection significantly increased ( P & lt ; 0.05 ) the contribution of transsulfuration to cysteine flux in both plasma and liver ( by 80 % ) and the contribution of transsulfuration to plasma methionine flux ( by 133 % ) .
	manualset3
100749	11	401208	13	NULL	NULL	0	NULL	by 133 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection significantly increased ( P & lt ; 0.05 ) the contribution of transsulfuration to cysteine flux in both plasma and liver ( by 80 % ) and the contribution of transsulfuration to plasma methionine flux ( by 133 % ) .
	manualset3
102520	12	401208	13	NULL	NULL	0	NULL	contribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection significantly increased ( P & lt ; 0.05 ) the contribution of transsulfuration to cysteine flux in both plasma and liver ( by 80 % ) and the contribution of transsulfuration to plasma methionine flux ( by 133 % ) .
	manualset3
100750	1	401209	13	NULL	NULL	0	NULL	Infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection was suspected , and we administered antibiotics and antifungal agents , while holding steroid administration .
	manualset3
100751	2	401209	13	NULL	NULL	0	NULL	antibiotics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection was suspected , and we administered antibiotics and antifungal agents , while holding steroid administration .
	manualset3
100752	3	401209	13	NULL	NULL	0	NULL	antifungal agents	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection was suspected , and we administered antibiotics and antifungal agents , while holding steroid administration .
	manualset3
100753	4	401209	13	NULL	NULL	0	NULL	steroid administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection was suspected , and we administered antibiotics and antifungal agents , while holding steroid administration .
	manualset3
100754	1	401210	13	NULL	NULL	0	NULL	Infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection with hepatitis C and the alcohol abuse that frequently accompanies it , impose major worldwide healthcare burdens .
	manualset3
100755	2	401210	13	NULL	NULL	0	NULL	hepatitis C	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection with hepatitis C and the alcohol abuse that frequently accompanies it , impose major worldwide healthcare burdens .
	manualset3
100756	3	401210	13	NULL	NULL	0	NULL	alcohol abuse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection with hepatitis C and the alcohol abuse that frequently accompanies it , impose major worldwide healthcare burdens .
	manualset3
100757	4	401210	13	NULL	NULL	0	NULL	worldwide	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection with hepatitis C and the alcohol abuse that frequently accompanies it , impose major worldwide healthcare burdens .
	manualset3
100758	5	401210	13	NULL	NULL	0	NULL	healthcare burdens	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection with hepatitis C and the alcohol abuse that frequently accompanies it , impose major worldwide healthcare burdens .
	manualset3
100759	1	401211	13	NULL	NULL	0	NULL	Infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection with parvovirus during pregnancy .
	manualset3
100760	2	401211	13	NULL	NULL	0	NULL	parvovirus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection with parvovirus during pregnancy .
	manualset3
100762	3	401211	13	NULL	NULL	0	NULL	pregnancy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infection with parvovirus during pregnancy .
	manualset3
100763	1	401212	13	NULL	NULL	0	NULL	Infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infections in the elderly are often accompanied by serious complications as bacteriemia ( pneumonia ) , frequent recurrence ( UTI ) , perforation and abscess ( abdominal infections ) and severe disability ( pressure ulcer infections ) .
	manualset3
100764	2	401212	13	NULL	NULL	0	NULL	elderly	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Infections in the elderly are often accompanied by serious complications as bacteriemia ( pneumonia ) , frequent recurrence ( UTI ) , perforation and abscess ( abdominal infections ) and severe disability ( pressure ulcer infections ) .
	manualset3
100765	3	401212	13	NULL	NULL	0	NULL	serious complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infections in the elderly are often accompanied by serious complications as bacteriemia ( pneumonia ) , frequent recurrence ( UTI ) , perforation and abscess ( abdominal infections ) and severe disability ( pressure ulcer infections ) .
	manualset3
100766	4	401212	13	NULL	NULL	0	NULL	bacteriemia ( pneumonia ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infections in the elderly are often accompanied by serious complications as bacteriemia ( pneumonia ) , frequent recurrence ( UTI ) , perforation and abscess ( abdominal infections ) and severe disability ( pressure ulcer infections ) .
	manualset3
100767	5	401212	13	NULL	NULL	0	NULL	frequent recurrence ( UTI )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infections in the elderly are often accompanied by serious complications as bacteriemia ( pneumonia ) , frequent recurrence ( UTI ) , perforation and abscess ( abdominal infections ) and severe disability ( pressure ulcer infections ) .
	manualset3
100768	6	401212	13	NULL	NULL	0	NULL	perforation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infections in the elderly are often accompanied by serious complications as bacteriemia ( pneumonia ) , frequent recurrence ( UTI ) , perforation and abscess ( abdominal infections ) and severe disability ( pressure ulcer infections ) .
	manualset3
100769	7	401212	13	NULL	NULL	0	NULL	abscess	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infections in the elderly are often accompanied by serious complications as bacteriemia ( pneumonia ) , frequent recurrence ( UTI ) , perforation and abscess ( abdominal infections ) and severe disability ( pressure ulcer infections ) .
	manualset3
100770	8	401212	13	NULL	NULL	0	NULL	abdominal infections 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infections in the elderly are often accompanied by serious complications as bacteriemia ( pneumonia ) , frequent recurrence ( UTI ) , perforation and abscess ( abdominal infections ) and severe disability ( pressure ulcer infections ) .
	manualset3
100771	9	401212	13	NULL	NULL	0	NULL	severe disability 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infections in the elderly are often accompanied by serious complications as bacteriemia ( pneumonia ) , frequent recurrence ( UTI ) , perforation and abscess ( abdominal infections ) and severe disability ( pressure ulcer infections ) .
	manualset3
100772	10	401212	13	NULL	NULL	0	NULL	pressure ulcer infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infections in the elderly are often accompanied by serious complications as bacteriemia ( pneumonia ) , frequent recurrence ( UTI ) , perforation and abscess ( abdominal infections ) and severe disability ( pressure ulcer infections ) .
	manualset3
100773	1	401213	13	NULL	NULL	0	NULL	206 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	206 of the 274 did not undergo hysteroscopy because of gynecological , psychological , or general contraindications , or failure of the patient to appear for follow-up .
	manualset3
100774	2	401213	13	NULL	NULL	0	NULL	274	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	206 of the 274 did not undergo hysteroscopy because of gynecological , psychological , or general contraindications , or failure of the patient to appear for follow-up .
	manualset3
100775	3	401213	13	NULL	NULL	0	NULL	hysteroscopy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	206 of the 274 did not undergo hysteroscopy because of gynecological , psychological , or general contraindications , or failure of the patient to appear for follow-up .
	manualset3
100776	4	401213	13	NULL	NULL	0	NULL	gynecological contraindications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	206 of the 274 did not undergo hysteroscopy because of gynecological , psychological , or general contraindications , or failure of the patient to appear for follow-up .
	manualset3
100777	5	401213	13	NULL	NULL	0	NULL	psychological contraindications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	206 of the 274 did not undergo hysteroscopy because of gynecological , psychological , or general contraindications , or failure of the patient to appear for follow-up .
	manualset3
100778	6	401213	13	NULL	NULL	0	NULL	general contraindications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	206 of the 274 did not undergo hysteroscopy because of gynecological , psychological , or general contraindications , or failure of the patient to appear for follow-up .
	manualset3
100779	7	401213	13	NULL	NULL	0	NULL	failure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	206 of the 274 did not undergo hysteroscopy because of gynecological , psychological , or general contraindications , or failure of the patient to appear for follow-up .
	manualset3
100780	8	401213	13	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	206 of the 274 did not undergo hysteroscopy because of gynecological , psychological , or general contraindications , or failure of the patient to appear for follow-up .
	manualset3
100781	9	401213	13	NULL	NULL	0	NULL	follow-up	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	206 of the 274 did not undergo hysteroscopy because of gynecological , psychological , or general contraindications , or failure of the patient to appear for follow-up .
	manualset3
100782	1	401214	13	NULL	NULL	0	NULL	Infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infections with hepatitis B virus ( HBV ) or hepatitis C virus ( HCV ) are associated with significant morbidity and mortality among patients with cancer , especially in patients with hematologic malignancies and those who undergo hematopoietic stem-cell transplantation .
	manualset3
100783	2	401214	13	NULL	NULL	0	NULL	hepatitis B virus ( HBV ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Infections with hepatitis B virus ( HBV ) or hepatitis C virus ( HCV ) are associated with significant morbidity and mortality among patients with cancer , especially in patients with hematologic malignancies and those who undergo hematopoietic stem-cell transplantation .
	manualset3
100784	3	401214	13	NULL	NULL	0	NULL	hepatitis C virus ( HCV ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Infections with hepatitis B virus ( HBV ) or hepatitis C virus ( HCV ) are associated with significant morbidity and mortality among patients with cancer , especially in patients with hematologic malignancies and those who undergo hematopoietic stem-cell transplantation .
	manualset3
100785	4	401214	13	NULL	NULL	0	NULL	morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infections with hepatitis B virus ( HBV ) or hepatitis C virus ( HCV ) are associated with significant morbidity and mortality among patients with cancer , especially in patients with hematologic malignancies and those who undergo hematopoietic stem-cell transplantation .
	manualset3
100786	5	401214	13	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infections with hepatitis B virus ( HBV ) or hepatitis C virus ( HCV ) are associated with significant morbidity and mortality among patients with cancer , especially in patients with hematologic malignancies and those who undergo hematopoietic stem-cell transplantation .
	manualset3
100787	6	401214	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Infections with hepatitis B virus ( HBV ) or hepatitis C virus ( HCV ) are associated with significant morbidity and mortality among patients with cancer , especially in patients with hematologic malignancies and those who undergo hematopoietic stem-cell transplantation .
	manualset3
100788	7	401214	13	NULL	NULL	0	NULL	cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Infections with hepatitis B virus ( HBV ) or hepatitis C virus ( HCV ) are associated with significant morbidity and mortality among patients with cancer , especially in patients with hematologic malignancies and those who undergo hematopoietic stem-cell transplantation .
	manualset3
100789	8	401214	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Infections with hepatitis B virus ( HBV ) or hepatitis C virus ( HCV ) are associated with significant morbidity and mortality among patients with cancer , especially in patients with hematologic malignancies and those who undergo hematopoietic stem-cell transplantation .
	manualset3
100790	9	401214	13	NULL	NULL	0	NULL	hematologic malignancies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infections with hepatitis B virus ( HBV ) or hepatitis C virus ( HCV ) are associated with significant morbidity and mortality among patients with cancer , especially in patients with hematologic malignancies and those who undergo hematopoietic stem-cell transplantation .
	manualset3
100791	10	401214	13	NULL	NULL	0	NULL	hematopoietic stem-cell transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Infections with hepatitis B virus ( HBV ) or hepatitis C virus ( HCV ) are associated with significant morbidity and mortality among patients with cancer , especially in patients with hematologic malignancies and those who undergo hematopoietic stem-cell transplantation .
	manualset3
100792	1	401215	13	NULL	NULL	0	NULL	Infectious virus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Infectious virus was detected earlier in plasma than in any of the mononuclear cell subpopulations .
	manualset3
100793	2	401215	13	NULL	NULL	0	NULL	plasma	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Infectious virus was detected earlier in plasma than in any of the mononuclear cell subpopulations .
	manualset3
100794	3	401215	13	NULL	NULL	0	NULL	mononuclear cell subpopulations	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Infectious virus was detected earlier in plasma than in any of the mononuclear cell subpopulations .
	manualset3
100795	1	401216	13	NULL	NULL	0	NULL	Infectivity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infectivity is instead characterised by both the number and sizes of the PrP ( Sc ) aggregates .
	manualset3
100796	2	401216	13	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Infectivity is instead characterised by both the number and sizes of the PrP ( Sc ) aggregates .
	manualset3
100797	3	401216	13	NULL	NULL	0	NULL	sizes	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Infectivity is instead characterised by both the number and sizes of the PrP ( Sc ) aggregates .
	manualset3
100798	4	401216	13	NULL	NULL	0	NULL	PrP ( Sc ) aggregates	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Infectivity is instead characterised by both the number and sizes of the PrP ( Sc ) aggregates .
	manualset3
100799	1	401217	13	NULL	NULL	0	NULL	Inferences 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inferences were drawn regarding the nature of chronic simple glaucoma and ocular hypertension and their management .
	manualset3
100800	2	401217	13	NULL	NULL	0	NULL	nature of chronic simple glaucoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inferences were drawn regarding the nature of chronic simple glaucoma and ocular hypertension and their management .
	manualset3
100801	3	401217	13	NULL	NULL	0	NULL	ocular hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inferences were drawn regarding the nature of chronic simple glaucoma and ocular hypertension and their management .
	manualset3
100802	4	401217	13	NULL	NULL	0	NULL	management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Inferences were drawn regarding the nature of chronic simple glaucoma and ocular hypertension and their management .
	manualset3
100803	1	401218	13	NULL	NULL	0	NULL	human population sizes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Inferring human population sizes , divergence times and rates of gene flow from mitochondrial , X and Y chromosome resequencing data .
	manualset3
100804	2	401218	13	NULL	NULL	0	NULL	divergence times	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Inferring human population sizes , divergence times and rates of gene flow from mitochondrial , X and Y chromosome resequencing data .
	manualset3
100805	3	401218	13	NULL	NULL	0	NULL	rates of gene flow	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Inferring human population sizes , divergence times and rates of gene flow from mitochondrial , X and Y chromosome resequencing data .
	manualset3
100806	4	401218	13	NULL	NULL	0	NULL	 mitochondrial resequencing data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Inferring human population sizes , divergence times and rates of gene flow from mitochondrial , X and Y chromosome resequencing data .
	manualset3
100807	5	401218	13	NULL	NULL	0	NULL	 X chromosome resequencing data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Inferring human population sizes , divergence times and rates of gene flow from mitochondrial , X and Y chromosome resequencing data .
	manualset3
100808	6	401218	13	NULL	NULL	0	NULL	Y chromosome resequencing data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Inferring human population sizes , divergence times and rates of gene flow from mitochondrial , X and Y chromosome resequencing data .
	manualset3
100809	1	401219	13	NULL	NULL	0	NULL	Infertile women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Infertile women associated with anovulation were treated by 50-150 mg of CC for five consecutive days in each treatment cycle .
	manualset3
100810	2	401219	13	NULL	NULL	0	NULL	anovulation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infertile women associated with anovulation were treated by 50-150 mg of CC for five consecutive days in each treatment cycle .
	manualset3
100811	3	401219	13	NULL	NULL	0	NULL	50-150 mg of CC	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Infertile women associated with anovulation were treated by 50-150 mg of CC for five consecutive days in each treatment cycle .
	manualset3
100812	4	401219	13	NULL	NULL	0	NULL	five consecutive days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Infertile women associated with anovulation were treated by 50-150 mg of CC for five consecutive days in each treatment cycle .
	manualset3
100813	5	401219	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Infertile women associated with anovulation were treated by 50-150 mg of CC for five consecutive days in each treatment cycle .
	manualset3
100814	6	401219	13	NULL	NULL	0	NULL	cycle	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Infertile women associated with anovulation were treated by 50-150 mg of CC for five consecutive days in each treatment cycle .
	manualset3
100815	1	401220	13	NULL	NULL	0	NULL	Infertile women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Infertile women without tubal obstruction had antibody titers similar to the control group with an odds ratio of 1.1 ( 95 % CI : 0.6-1 .9 ) .
	manualset3
100816	2	401220	13	NULL	NULL	0	NULL	tubal obstruction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infertile women without tubal obstruction had antibody titers similar to the control group with an odds ratio of 1.1 ( 95 % CI : 0.6-1 .9 ) .
	manualset3
100817	3	401220	13	NULL	NULL	0	NULL	antibody titers	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Infertile women without tubal obstruction had antibody titers similar to the control group with an odds ratio of 1.1 ( 95 % CI : 0.6-1 .9 ) .
	manualset3
100818	4	401220	13	NULL	NULL	0	NULL	control group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Infertile women without tubal obstruction had antibody titers similar to the control group with an odds ratio of 1.1 ( 95 % CI : 0.6-1 .9 ) .
	manualset3
100819	5	401220	13	NULL	NULL	0	NULL	odds ratio of 1.1 ( 95 % CI : 0.6-1 .9 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Infertile women without tubal obstruction had antibody titers similar to the control group with an odds ratio of 1.1 ( 95 % CI : 0.6-1 .9 ) .
	manualset3
100820	1	401221	13	NULL	NULL	0	NULL	Infertility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infertility is recognized as an important clinical and social issue , because of the common occurrence and therapeutical difficulties .
	manualset3
100821	2	401221	13	NULL	NULL	0	NULL	clinical issue	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infertility is recognized as an important clinical and social issue , because of the common occurrence and therapeutical difficulties .
	manualset3
100822	3	401221	13	NULL	NULL	0	NULL	social issue	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infertility is recognized as an important clinical and social issue , because of the common occurrence and therapeutical difficulties .
	manualset3
100823	4	401221	13	NULL	NULL	0	NULL	common occurrence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infertility is recognized as an important clinical and social issue , because of the common occurrence and therapeutical difficulties .
	manualset3
100824	5	401221	13	NULL	NULL	0	NULL	 therapeutical difficulties	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infertility is recognized as an important clinical and social issue , because of the common occurrence and therapeutical difficulties .
	manualset3
100825	1	401222	13	NULL	NULL	0	NULL	Inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammation and oxidant-stress in beta-thalassemia patients treated with iron chelators deferasirox ( ICL670 ) or deferoxamine : an ancillary study of the Novartis CICL670A0107 trial .
	manualset3
100826	2	401222	13	NULL	NULL	0	NULL	oxidant-stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammation and oxidant-stress in beta-thalassemia patients treated with iron chelators deferasirox ( ICL670 ) or deferoxamine : an ancillary study of the Novartis CICL670A0107 trial .
	manualset3
100827	3	401222	13	NULL	NULL	0	NULL	 beta-thalassemia patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammation and oxidant-stress in beta-thalassemia patients treated with iron chelators deferasirox ( ICL670 ) or deferoxamine : an ancillary study of the Novartis CICL670A0107 trial .
	manualset3
100828	4	401222	13	NULL	NULL	0	NULL	iron chelators 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammation and oxidant-stress in beta-thalassemia patients treated with iron chelators deferasirox ( ICL670 ) or deferoxamine : an ancillary study of the Novartis CICL670A0107 trial .
	manualset3
100829	5	401222	13	NULL	NULL	0	NULL	deferasirox ( ICL670 )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammation and oxidant-stress in beta-thalassemia patients treated with iron chelators deferasirox ( ICL670 ) or deferoxamine : an ancillary study of the Novartis CICL670A0107 trial .
	manualset3
100830	6	401222	13	NULL	NULL	0	NULL	deferoxamine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammation and oxidant-stress in beta-thalassemia patients treated with iron chelators deferasirox ( ICL670 ) or deferoxamine : an ancillary study of the Novartis CICL670A0107 trial .
	manualset3
100831	7	401222	13	NULL	NULL	0	NULL	ancillary study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammation and oxidant-stress in beta-thalassemia patients treated with iron chelators deferasirox ( ICL670 ) or deferoxamine : an ancillary study of the Novartis CICL670A0107 trial .
	manualset3
100832	8	401222	13	NULL	NULL	0	NULL	Novartis CICL670A0107 trial 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammation and oxidant-stress in beta-thalassemia patients treated with iron chelators deferasirox ( ICL670 ) or deferoxamine : an ancillary study of the Novartis CICL670A0107 trial .
	manualset3
100833	1	401223	13	NULL	NULL	0	NULL	Inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammation has a pivotal role in the development of atherosclerosis and acute activation of the vascular wall with consecutive local thrombosis and altered vasomotion .
	manualset3
100834	2	401223	13	NULL	NULL	0	NULL	pivotal role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammation has a pivotal role in the development of atherosclerosis and acute activation of the vascular wall with consecutive local thrombosis and altered vasomotion .
	manualset3
100835	3	401223	13	NULL	NULL	0	NULL	development	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammation has a pivotal role in the development of atherosclerosis and acute activation of the vascular wall with consecutive local thrombosis and altered vasomotion .
	manualset3
100836	4	401223	13	NULL	NULL	0	NULL	atherosclerosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammation has a pivotal role in the development of atherosclerosis and acute activation of the vascular wall with consecutive local thrombosis and altered vasomotion .
	manualset3
100837	5	401223	13	NULL	NULL	0	NULL	acute activation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammation has a pivotal role in the development of atherosclerosis and acute activation of the vascular wall with consecutive local thrombosis and altered vasomotion .
	manualset3
100838	6	401223	13	NULL	NULL	0	NULL	vascular wall	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammation has a pivotal role in the development of atherosclerosis and acute activation of the vascular wall with consecutive local thrombosis and altered vasomotion .
	manualset3
100839	7	401223	13	NULL	NULL	0	NULL	local thrombosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammation has a pivotal role in the development of atherosclerosis and acute activation of the vascular wall with consecutive local thrombosis and altered vasomotion .
	manualset3
100840	8	401223	13	NULL	NULL	0	NULL	vasomotion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammation has a pivotal role in the development of atherosclerosis and acute activation of the vascular wall with consecutive local thrombosis and altered vasomotion .
	manualset3
100841	1	401224	13	NULL	NULL	0	NULL	Inflammations 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammations of the digestive tract ( esophagus , stomach and duodenum ) in school-age children ) .
	manualset3
100842	2	401224	13	NULL	NULL	0	NULL	digestive tract 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammations of the digestive tract ( esophagus , stomach and duodenum ) in school-age children ) .
	manualset3
100843	3	401224	13	NULL	NULL	0	NULL	esophagus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammations of the digestive tract ( esophagus , stomach and duodenum ) in school-age children ) .
	manualset3
100844	4	401224	13	NULL	NULL	0	NULL	stomach	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammations of the digestive tract ( esophagus , stomach and duodenum ) in school-age children ) .
	manualset3
100845	5	401224	13	NULL	NULL	0	NULL	duodenum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammations of the digestive tract ( esophagus , stomach and duodenum ) in school-age children ) .
	manualset3
100846	6	401224	13	NULL	NULL	0	NULL	school-age children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammations of the digestive tract ( esophagus , stomach and duodenum ) in school-age children ) .
	manualset3
100847	1	401225	13	NULL	NULL	0	NULL	Inflammatory bowel disease ( IBD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammatory bowel disease ( IBD ) is now recognized as a common chronic disease affecting children and adolescents .
	manualset3
100848	2	401225	13	NULL	NULL	0	NULL	common chronic disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammatory bowel disease ( IBD ) is now recognized as a common chronic disease affecting children and adolescents .
	manualset3
100849	3	401225	13	NULL	NULL	0	NULL	 children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammatory bowel disease ( IBD ) is now recognized as a common chronic disease affecting children and adolescents .
	manualset3
100850	4	401225	13	NULL	NULL	0	NULL	adolescents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammatory bowel disease ( IBD ) is now recognized as a common chronic disease affecting children and adolescents .
	manualset3
100851	1	401226	13	NULL	NULL	0	NULL	Inflammatory cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammatory cells may be associated with malignant transformation and tumor regression .
	manualset3
100852	2	401226	13	NULL	NULL	0	NULL	malignant transformation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammatory cells may be associated with malignant transformation and tumor regression .
	manualset3
100853	3	401226	13	NULL	NULL	0	NULL	tumor regression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammatory cells may be associated with malignant transformation and tumor regression .
	manualset3
100854	1	401227	13	NULL	NULL	0	NULL	Inflammatory conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammatory conditions , tumors and aseptic bone necrosis are demonstrated with a high degree of sensitivity .
	manualset3
100855	2	401227	13	NULL	NULL	0	NULL	tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammatory conditions , tumors and aseptic bone necrosis are demonstrated with a high degree of sensitivity .
	manualset3
100856	3	401227	13	NULL	NULL	0	NULL	aseptic bone necrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammatory conditions , tumors and aseptic bone necrosis are demonstrated with a high degree of sensitivity .
	manualset3
100857	4	401227	13	NULL	NULL	0	NULL	high degree of sensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammatory conditions , tumors and aseptic bone necrosis are demonstrated with a high degree of sensitivity .
	manualset3
100858	1	401228	13	NULL	NULL	0	NULL	Inflammatory mediators	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammatory mediators are operative in the pathogenesis of the most common forms of heart disease .
	manualset3
100859	2	401228	13	NULL	NULL	0	NULL	pathogenesis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammatory mediators are operative in the pathogenesis of the most common forms of heart disease .
	manualset3
100860	3	401228	13	NULL	NULL	0	NULL	common forms of heart disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammatory mediators are operative in the pathogenesis of the most common forms of heart disease .
	manualset3
100861	1	401229	13	NULL	NULL	0	NULL	Inflammatory mediators	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammatory mediators or catecholamine amplifying diabetic RBC adhesion may aggravate endothelial cell damages .
	manualset3
100862	2	401229	13	NULL	NULL	0	NULL	catecholamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammatory mediators or catecholamine amplifying diabetic RBC adhesion may aggravate endothelial cell damages .
	manualset3
100863	3	401229	13	NULL	NULL	0	NULL	diabetic RBC adhesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammatory mediators or catecholamine amplifying diabetic RBC adhesion may aggravate endothelial cell damages .
	manualset3
100864	4	401229	13	NULL	NULL	0	NULL	endothelial cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammatory mediators or catecholamine amplifying diabetic RBC adhesion may aggravate endothelial cell damages .
	manualset3
100865	5	401229	13	NULL	NULL	0	NULL	damages	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammatory mediators or catecholamine amplifying diabetic RBC adhesion may aggravate endothelial cell damages .
	manualset3
100866	1	401230	13	NULL	NULL	0	NULL	Inflation pressures	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflation pressures of +40 and +50 cm H2O caused a marked but transient bradycardia along with a ( probably spurious ) short-lasting fall to 89 % mean arterial oxygen saturation ( SaO2 ) .
	manualset3
100867	2	401230	13	NULL	NULL	0	NULL	+40 cm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflation pressures of +40 and +50 cm H2O caused a marked but transient bradycardia along with a ( probably spurious ) short-lasting fall to 89 % mean arterial oxygen saturation ( SaO2 ) .
	manualset3
100868	3	401230	13	NULL	NULL	0	NULL	+50 cm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflation pressures of +40 and +50 cm H2O caused a marked but transient bradycardia along with a ( probably spurious ) short-lasting fall to 89 % mean arterial oxygen saturation ( SaO2 ) .
	manualset3
100869	4	401230	13	NULL	NULL	0	NULL	H2O	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflation pressures of +40 and +50 cm H2O caused a marked but transient bradycardia along with a ( probably spurious ) short-lasting fall to 89 % mean arterial oxygen saturation ( SaO2 ) .
	manualset3
100870	5	401230	13	NULL	NULL	0	NULL	transient bradycardia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflation pressures of +40 and +50 cm H2O caused a marked but transient bradycardia along with a ( probably spurious ) short-lasting fall to 89 % mean arterial oxygen saturation ( SaO2 ) .
	manualset3
100871	6	401230	13	NULL	NULL	0	NULL	short-lasting fall 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflation pressures of +40 and +50 cm H2O caused a marked but transient bradycardia along with a ( probably spurious ) short-lasting fall to 89 % mean arterial oxygen saturation ( SaO2 ) .
	manualset3
100872	7	401230	13	NULL	NULL	0	NULL	89 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflation pressures of +40 and +50 cm H2O caused a marked but transient bradycardia along with a ( probably spurious ) short-lasting fall to 89 % mean arterial oxygen saturation ( SaO2 ) .
	manualset3
100873	8	401230	13	NULL	NULL	0	NULL	mean arterial oxygen saturation ( SaO2 ) 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflation pressures of +40 and +50 cm H2O caused a marked but transient bradycardia along with a ( probably spurious ) short-lasting fall to 89 % mean arterial oxygen saturation ( SaO2 ) .
	manualset3
100882	1	401231	13	NULL	NULL	0	NULL	212	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	212 Sucklings affected with bronchiolitis were evaluated monitoring values of haematic gases and acid-base balance .
	manualset3
100883	2	401231	13	NULL	NULL	0	NULL	Sucklings	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	212 Sucklings affected with bronchiolitis were evaluated monitoring values of haematic gases and acid-base balance .
	manualset3
100884	3	401231	13	NULL	NULL	0	NULL	 bronchiolitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	212 Sucklings affected with bronchiolitis were evaluated monitoring values of haematic gases and acid-base balance .
	manualset3
100885	4	401231	13	NULL	NULL	0	NULL	monitoring values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	212 Sucklings affected with bronchiolitis were evaluated monitoring values of haematic gases and acid-base balance .
	manualset3
100886	5	401231	13	NULL	NULL	0	NULL	 haematic gases	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	212 Sucklings affected with bronchiolitis were evaluated monitoring values of haematic gases and acid-base balance .
	manualset3
100887	6	401231	13	NULL	NULL	0	NULL	acid-base balance 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	212 Sucklings affected with bronchiolitis were evaluated monitoring values of haematic gases and acid-base balance .
	manualset3
101033	1	401232	13	NULL	NULL	0	NULL	Inflow 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflow of external medium to the nuclei during dissociation of the myosin from the perinuclear F-actin may be due to colloidal osmosis depending on other macromolecular components of the karyoplasm .
	manualset3
101034	2	401232	13	NULL	NULL	0	NULL	external medium	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflow of external medium to the nuclei during dissociation of the myosin from the perinuclear F-actin may be due to colloidal osmosis depending on other macromolecular components of the karyoplasm .
	manualset3
101035	3	401232	13	NULL	NULL	0	NULL	nuclei	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflow of external medium to the nuclei during dissociation of the myosin from the perinuclear F-actin may be due to colloidal osmosis depending on other macromolecular components of the karyoplasm .
	manualset3
101036	4	401232	13	NULL	NULL	0	NULL	dissociation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflow of external medium to the nuclei during dissociation of the myosin from the perinuclear F-actin may be due to colloidal osmosis depending on other macromolecular components of the karyoplasm .
	manualset3
101037	5	401232	13	NULL	NULL	0	NULL	myosin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflow of external medium to the nuclei during dissociation of the myosin from the perinuclear F-actin may be due to colloidal osmosis depending on other macromolecular components of the karyoplasm .
	manualset3
101038	6	401232	13	NULL	NULL	0	NULL	perinuclear F-actin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflow of external medium to the nuclei during dissociation of the myosin from the perinuclear F-actin may be due to colloidal osmosis depending on other macromolecular components of the karyoplasm .
	manualset3
101039	7	401232	13	NULL	NULL	0	NULL	colloidal osmosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflow of external medium to the nuclei during dissociation of the myosin from the perinuclear F-actin may be due to colloidal osmosis depending on other macromolecular components of the karyoplasm .
	manualset3
101040	8	401232	13	NULL	NULL	0	NULL	macromolecular components	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflow of external medium to the nuclei during dissociation of the myosin from the perinuclear F-actin may be due to colloidal osmosis depending on other macromolecular components of the karyoplasm .
	manualset3
101041	9	401232	13	NULL	NULL	0	NULL	karyoplasm	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflow of external medium to the nuclei during dissociation of the myosin from the perinuclear F-actin may be due to colloidal osmosis depending on other macromolecular components of the karyoplasm .
	manualset3
101042	1	401233	13	NULL	NULL	0	NULL	Influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of P2O5 on crystallinity of apatite formed in vitro on surface of bioactive glasses .
	manualset3
101043	2	401233	13	NULL	NULL	0	NULL	P2O5	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of P2O5 on crystallinity of apatite formed in vitro on surface of bioactive glasses .
	manualset3
101044	3	401233	13	NULL	NULL	0	NULL	crystallinity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of P2O5 on crystallinity of apatite formed in vitro on surface of bioactive glasses .
	manualset3
101045	4	401233	13	NULL	NULL	0	NULL	 apatite 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of P2O5 on crystallinity of apatite formed in vitro on surface of bioactive glasses .
	manualset3
101046	5	401233	13	NULL	NULL	0	NULL	surface of bioactive glasses	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of P2O5 on crystallinity of apatite formed in vitro on surface of bioactive glasses .
	manualset3
101047	1	401234	13	NULL	NULL	NULL	NULL	Influence	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Influence of a serotonin - and dopamine-rich diet on platelet serotonin content and urinary excretion of biogenic amines and their metabolites .
	manualset3
101048	2	401234	13	NULL	NULL	0	NULL	serotonin-rich diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of a serotonin - and dopamine-rich diet on platelet serotonin content and urinary excretion of biogenic amines and their metabolites .
	manualset3
101049	3	401234	13	NULL	NULL	0	NULL	dopamine-rich diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of a serotonin - and dopamine-rich diet on platelet serotonin content and urinary excretion of biogenic amines and their metabolites .
	manualset3
101050	4	401234	13	NULL	NULL	0	NULL	platelet serotonin content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of a serotonin - and dopamine-rich diet on platelet serotonin content and urinary excretion of biogenic amines and their metabolites .
	manualset3
101051	5	401234	13	NULL	NULL	0	NULL	urinary excretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of a serotonin - and dopamine-rich diet on platelet serotonin content and urinary excretion of biogenic amines and their metabolites .
	manualset3
101052	6	401234	13	NULL	NULL	0	NULL	biogenic amines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of a serotonin - and dopamine-rich diet on platelet serotonin content and urinary excretion of biogenic amines and their metabolites .
	manualset3
101053	7	401234	13	NULL	NULL	0	NULL	metabolites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of a serotonin - and dopamine-rich diet on platelet serotonin content and urinary excretion of biogenic amines and their metabolites .
	manualset3
101054	1	401235	13	NULL	NULL	0	NULL	Influence of age	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of age on the pharmacokinetics and pharmacodynamics of ximelagatran , an oral direct thrombin inhibitor .
	manualset3
101055	2	401235	13	NULL	NULL	0	NULL	pharmacokinetics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of age on the pharmacokinetics and pharmacodynamics of ximelagatran , an oral direct thrombin inhibitor .
	manualset3
101056	3	401235	13	NULL	NULL	0	NULL	pharmacodynamics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of age on the pharmacokinetics and pharmacodynamics of ximelagatran , an oral direct thrombin inhibitor .
	manualset3
101057	4	401235	13	NULL	NULL	0	NULL	ximelagatran	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of age on the pharmacokinetics and pharmacodynamics of ximelagatran , an oral direct thrombin inhibitor .
	manualset3
101058	5	401235	13	NULL	NULL	0	NULL	thrombin inhibitor	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of age on the pharmacokinetics and pharmacodynamics of ximelagatran , an oral direct thrombin inhibitor .
	manualset3
101059	1	401236	13	NULL	NULL	0	NULL	Influence	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of an ER-retention signal on the N-glycosylation of recombinant human - L-iduronidase generated in seeds of Arabidopsis .
	manualset3
101060	2	401236	13	NULL	NULL	0	NULL	ER-retention signal 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of an ER-retention signal on the N-glycosylation of recombinant human - L-iduronidase generated in seeds of Arabidopsis .
	manualset3
101061	3	401236	13	NULL	NULL	0	NULL	N-glycosylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of an ER-retention signal on the N-glycosylation of recombinant human - L-iduronidase generated in seeds of Arabidopsis .
	manualset3
101062	4	401236	13	NULL	NULL	0	NULL	 recombinant human - L-iduronidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of an ER-retention signal on the N-glycosylation of recombinant human - L-iduronidase generated in seeds of Arabidopsis .
	manualset3
101063	5	401236	13	NULL	NULL	0	NULL	seeds	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of an ER-retention signal on the N-glycosylation of recombinant human - L-iduronidase generated in seeds of Arabidopsis .
	manualset3
101064	6	401236	13	NULL	NULL	0	NULL	Arabidopsis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of an ER-retention signal on the N-glycosylation of recombinant human - L-iduronidase generated in seeds of Arabidopsis .
	manualset3
101065	1	401237	13	NULL	NULL	0	NULL	Influence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of chronic aminophylline on the anticonvulsant efficacy of phenobarbital and valproate in mice .
	manualset3
101066	2	401237	13	NULL	NULL	0	NULL	chronic aminophylline	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of chronic aminophylline on the anticonvulsant efficacy of phenobarbital and valproate in mice .
	manualset3
101067	3	401237	13	NULL	NULL	0	NULL	anticonvulsant efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of chronic aminophylline on the anticonvulsant efficacy of phenobarbital and valproate in mice .
	manualset3
101068	4	401237	13	NULL	NULL	0	NULL	phenobarbital	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of chronic aminophylline on the anticonvulsant efficacy of phenobarbital and valproate in mice .
	manualset3
101069	5	401237	13	NULL	NULL	0	NULL	valproate	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of chronic aminophylline on the anticonvulsant efficacy of phenobarbital and valproate in mice .
	manualset3
101070	6	401237	13	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of chronic aminophylline on the anticonvulsant efficacy of phenobarbital and valproate in mice .
	manualset3
101071	1	401238	13	NULL	NULL	0	NULL	Influence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of circumcision technique on frequency of urinary tract infections in neonates .
	manualset3
101072	2	401238	13	NULL	NULL	0	NULL	circumcision technique	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of circumcision technique on frequency of urinary tract infections in neonates .
	manualset3
101073	3	401238	13	NULL	NULL	0	NULL	frequency 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of circumcision technique on frequency of urinary tract infections in neonates .
	manualset3
101074	4	401238	13	NULL	NULL	0	NULL	urinary tract infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of circumcision technique on frequency of urinary tract infections in neonates .
	manualset3
101075	5	401238	13	NULL	NULL	0	NULL	neonates	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of circumcision technique on frequency of urinary tract infections in neonates .
	manualset3
101076	1	401239	13	NULL	NULL	0	NULL	Influence	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of endotoxin on arachidonate metabolism in isolated rabbit peritoneum .
	manualset3
101077	2	401239	13	NULL	NULL	0	NULL	endotoxin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of endotoxin on arachidonate metabolism in isolated rabbit peritoneum .
	manualset3
101078	3	401239	13	NULL	NULL	0	NULL	arachidonate metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of endotoxin on arachidonate metabolism in isolated rabbit peritoneum .
	manualset3
101079	4	401239	13	NULL	NULL	0	NULL	rabbit peritoneum 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of endotoxin on arachidonate metabolism in isolated rabbit peritoneum .
	manualset3
101080	1	401240	13	NULL	NULL	0	NULL	229E	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	229E replicated in human WI-38 cells but not in three mouse cell lines tested ( RAG , LM/TK - , and A9 ) .
	manualset3
101081	2	401240	13	NULL	NULL	0	NULL	human WI-38 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	229E replicated in human WI-38 cells but not in three mouse cell lines tested ( RAG , LM/TK - , and A9 ) .
	manualset3
101082	3	401240	13	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	229E replicated in human WI-38 cells but not in three mouse cell lines tested ( RAG , LM/TK - , and A9 ) .
	manualset3
101083	4	401240	13	NULL	NULL	0	NULL	 mouse cell lines 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	229E replicated in human WI-38 cells but not in three mouse cell lines tested ( RAG , LM/TK - , and A9 ) .
	manualset3
101084	5	401240	13	NULL	NULL	0	NULL	RAG	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	229E replicated in human WI-38 cells but not in three mouse cell lines tested ( RAG , LM/TK - , and A9 ) .
	manualset3
101085	6	401240	13	NULL	NULL	0	NULL	LM/TK	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	229E replicated in human WI-38 cells but not in three mouse cell lines tested ( RAG , LM/TK - , and A9 ) .
	manualset3
101086	7	401240	13	NULL	NULL	0	NULL	A9	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	229E replicated in human WI-38 cells but not in three mouse cell lines tested ( RAG , LM/TK - , and A9 ) .
	manualset3
101088	1	401241	13	NULL	NULL	0	NULL	Influence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of environmental temperature on experimental infection of redfin perch ( Perca fluviatilis ) and rainbow trout ( Oncorhynchus mykiss ) with epizootic hematopoietic necrosis virus , an Australian iridovirus .
	manualset3
101089	2	401241	13	NULL	NULL	0	NULL	environmental temperature	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of environmental temperature on experimental infection of redfin perch ( Perca fluviatilis ) and rainbow trout ( Oncorhynchus mykiss ) with epizootic hematopoietic necrosis virus , an Australian iridovirus .
	manualset3
101090	3	401241	13	NULL	NULL	0	NULL	experimental infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of environmental temperature on experimental infection of redfin perch ( Perca fluviatilis ) and rainbow trout ( Oncorhynchus mykiss ) with epizootic hematopoietic necrosis virus , an Australian iridovirus .
	manualset3
101091	4	401241	13	NULL	NULL	0	NULL	redfin perch	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of environmental temperature on experimental infection of redfin perch ( Perca fluviatilis ) and rainbow trout ( Oncorhynchus mykiss ) with epizootic hematopoietic necrosis virus , an Australian iridovirus .
	manualset3
101092	5	401241	13	NULL	NULL	0	NULL	Perca fluviatilis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of environmental temperature on experimental infection of redfin perch ( Perca fluviatilis ) and rainbow trout ( Oncorhynchus mykiss ) with epizootic hematopoietic necrosis virus , an Australian iridovirus .
	manualset3
101093	6	401241	13	NULL	NULL	0	NULL	rainbow trout	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of environmental temperature on experimental infection of redfin perch ( Perca fluviatilis ) and rainbow trout ( Oncorhynchus mykiss ) with epizootic hematopoietic necrosis virus , an Australian iridovirus .
	manualset3
101094	7	401241	13	NULL	NULL	0	NULL	Oncorhynchus mykiss	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of environmental temperature on experimental infection of redfin perch ( Perca fluviatilis ) and rainbow trout ( Oncorhynchus mykiss ) with epizootic hematopoietic necrosis virus , an Australian iridovirus .
	manualset3
101095	8	401241	13	NULL	NULL	0	NULL	epizootic hematopoietic necrosis virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of environmental temperature on experimental infection of redfin perch ( Perca fluviatilis ) and rainbow trout ( Oncorhynchus mykiss ) with epizootic hematopoietic necrosis virus , an Australian iridovirus .
	manualset3
101096	9	401241	13	NULL	NULL	0	NULL	Australian iridovirus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of environmental temperature on experimental infection of redfin perch ( Perca fluviatilis ) and rainbow trout ( Oncorhynchus mykiss ) with epizootic hematopoietic necrosis virus , an Australian iridovirus .
	manualset3
101097	1	401242	13	NULL	NULL	0	NULL	Influence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of hypothyroidism induced by thiamazole on the toxic interaction between propranolol and disopyramide in chick embryos .
	manualset3
101098	2	401242	13	NULL	NULL	0	NULL	hypothyroidism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of hypothyroidism induced by thiamazole on the toxic interaction between propranolol and disopyramide in chick embryos .
	manualset3
101099	3	401242	13	NULL	NULL	0	NULL	thiamazole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of hypothyroidism induced by thiamazole on the toxic interaction between propranolol and disopyramide in chick embryos .
	manualset3
101100	4	401242	13	NULL	NULL	0	NULL	 toxic interaction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of hypothyroidism induced by thiamazole on the toxic interaction between propranolol and disopyramide in chick embryos .
	manualset3
101101	5	401242	13	NULL	NULL	0	NULL	propranolol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of hypothyroidism induced by thiamazole on the toxic interaction between propranolol and disopyramide in chick embryos .
	manualset3
101102	6	401242	13	NULL	NULL	0	NULL	disopyramide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of hypothyroidism induced by thiamazole on the toxic interaction between propranolol and disopyramide in chick embryos .
	manualset3
101103	7	401242	13	NULL	NULL	0	NULL	chick embryos	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of hypothyroidism induced by thiamazole on the toxic interaction between propranolol and disopyramide in chick embryos .
	manualset3
101104	1	401243	13	NULL	NULL	0	NULL	Influence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of lansoprazole and rabeprazole on mycophenolic acid pharmacokinetics one year after renal transplantation .
	manualset3
101105	2	401243	13	NULL	NULL	0	NULL	lansoprazole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of lansoprazole and rabeprazole on mycophenolic acid pharmacokinetics one year after renal transplantation .
	manualset3
101106	3	401243	13	NULL	NULL	0	NULL	rabeprazole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of lansoprazole and rabeprazole on mycophenolic acid pharmacokinetics one year after renal transplantation .
	manualset3
101107	4	401243	13	NULL	NULL	0	NULL	mycophenolic acid pharmacokinetics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of lansoprazole and rabeprazole on mycophenolic acid pharmacokinetics one year after renal transplantation .
	manualset3
101108	5	401243	13	NULL	NULL	0	NULL	one year	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of lansoprazole and rabeprazole on mycophenolic acid pharmacokinetics one year after renal transplantation .
	manualset3
101109	6	401243	13	NULL	NULL	0	NULL	renal transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of lansoprazole and rabeprazole on mycophenolic acid pharmacokinetics one year after renal transplantation .
	manualset3
101110	1	401244	13	NULL	NULL	0	NULL	Influence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of maternal hypoxia on fetal tissue ascorbate levels .
	manualset3
101111	2	401244	13	NULL	NULL	0	NULL	maternal hypoxia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of maternal hypoxia on fetal tissue ascorbate levels .
	manualset3
101112	3	401244	13	NULL	NULL	0	NULL	fetal tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of maternal hypoxia on fetal tissue ascorbate levels .
	manualset3
101113	4	401244	13	NULL	NULL	0	NULL	ascorbate levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of maternal hypoxia on fetal tissue ascorbate levels .
	manualset3
101114	1	401245	13	NULL	NULL	0	NULL	Influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of operational parameters and kinetics analysis on the photocatalytic reduction of Cr ( VI ) by immobilized ZnO .
	manualset3
101115	2	401245	13	NULL	NULL	0	NULL	operational parameters	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of operational parameters and kinetics analysis on the photocatalytic reduction of Cr ( VI ) by immobilized ZnO .
	manualset3
101116	3	401245	13	NULL	NULL	0	NULL	kinetics analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of operational parameters and kinetics analysis on the photocatalytic reduction of Cr ( VI ) by immobilized ZnO .
	manualset3
101117	4	401245	13	NULL	NULL	0	NULL	photocatalytic reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of operational parameters and kinetics analysis on the photocatalytic reduction of Cr ( VI ) by immobilized ZnO .
	manualset3
101118	5	401245	13	NULL	NULL	0	NULL	Cr ( VI )	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of operational parameters and kinetics analysis on the photocatalytic reduction of Cr ( VI ) by immobilized ZnO .
	manualset3
101119	6	401245	13	NULL	NULL	0	NULL	ZnO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of operational parameters and kinetics analysis on the photocatalytic reduction of Cr ( VI ) by immobilized ZnO .
	manualset3
101120	1	401246	13	NULL	NULL	0	NULL	Influence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of phenytoin on cytoskeletal organization and cell viability of immortalized mouse hippocampal neurons .
	manualset3
101121	2	401246	13	NULL	NULL	0	NULL	 phenytoin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of phenytoin on cytoskeletal organization and cell viability of immortalized mouse hippocampal neurons .
	manualset3
101122	3	401246	13	NULL	NULL	0	NULL	cytoskeletal organization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of phenytoin on cytoskeletal organization and cell viability of immortalized mouse hippocampal neurons .
	manualset3
101123	4	401246	13	NULL	NULL	0	NULL	cell viability 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of phenytoin on cytoskeletal organization and cell viability of immortalized mouse hippocampal neurons .
	manualset3
101124	5	401246	13	NULL	NULL	0	NULL	 mouse hippocampal neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of phenytoin on cytoskeletal organization and cell viability of immortalized mouse hippocampal neurons .
	manualset3
101125	1	401247	13	NULL	NULL	0	NULL	Influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of porosity on the mechanical resistance of hydroxyapatite ceramics under compressive stress .
	manualset3
101126	2	401247	13	NULL	NULL	0	NULL	porosity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of porosity on the mechanical resistance of hydroxyapatite ceramics under compressive stress .
	manualset3
101127	3	401247	13	NULL	NULL	0	NULL	mechanical resistance 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of porosity on the mechanical resistance of hydroxyapatite ceramics under compressive stress .
	manualset3
101128	4	401247	13	NULL	NULL	0	NULL	hydroxyapatite ceramics	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of porosity on the mechanical resistance of hydroxyapatite ceramics under compressive stress .
	manualset3
101129	5	401247	13	NULL	NULL	0	NULL	compressive stress	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of porosity on the mechanical resistance of hydroxyapatite ceramics under compressive stress .
	manualset3
101130	1	401248	13	NULL	NULL	0	NULL	Influence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of sympathomimetic and sympatholytic drugs on the physiological and pharmacological actions of enteramine .
	manualset3
101131	2	401248	13	NULL	NULL	0	NULL	sympathomimetic drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of sympathomimetic and sympatholytic drugs on the physiological and pharmacological actions of enteramine .
	manualset3
101132	3	401248	13	NULL	NULL	0	NULL	sympatholytic drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of sympathomimetic and sympatholytic drugs on the physiological and pharmacological actions of enteramine .
	manualset3
101133	4	401248	13	NULL	NULL	0	NULL	physiological actions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of sympathomimetic and sympatholytic drugs on the physiological and pharmacological actions of enteramine .
	manualset3
101134	5	401248	13	NULL	NULL	0	NULL	pharmacological actions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of sympathomimetic and sympatholytic drugs on the physiological and pharmacological actions of enteramine .
	manualset3
101135	6	401248	13	NULL	NULL	0	NULL	enteramine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of sympathomimetic and sympatholytic drugs on the physiological and pharmacological actions of enteramine .
	manualset3
101136	1	401249	13	NULL	NULL	0	NULL	Influence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of the individual B6-vitamin factors on the intestinal absorption of L-methionine .
	manualset3
101137	2	401249	13	NULL	NULL	0	NULL	B6-vitamin factors	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of the individual B6-vitamin factors on the intestinal absorption of L-methionine .
	manualset3
101138	3	401249	13	NULL	NULL	0	NULL	intestinal absorption 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of the individual B6-vitamin factors on the intestinal absorption of L-methionine .
	manualset3
101139	4	401249	13	NULL	NULL	0	NULL	L-methionine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of the individual B6-vitamin factors on the intestinal absorption of L-methionine .
	manualset3
101140	1	401250	13	NULL	NULL	0	NULL	Influence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of the length of the small bowel graft on the severity of graft versus host disease .
	manualset3
101141	2	401250	13	NULL	NULL	0	NULL	length 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of the length of the small bowel graft on the severity of graft versus host disease .
	manualset3
101142	3	401250	13	NULL	NULL	0	NULL	small bowel graft 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of the length of the small bowel graft on the severity of graft versus host disease .
	manualset3
101143	4	401250	13	NULL	NULL	0	NULL	 severity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of the length of the small bowel graft on the severity of graft versus host disease .
	manualset3
101144	5	401250	13	NULL	NULL	0	NULL	graft versus host disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of the length of the small bowel graft on the severity of graft versus host disease .
	manualset3
101145	1	401251	13	NULL	NULL	0	NULL	237 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	237 patients who completed induction CT + RT and were classified as responders ( complete response + partial response ) were randomly assigned to arm 1 : low dose nIFN-alpha ( 91 patients ) ; arm 2 : maintenance CT , six cycles of CAP ( cyclophosphamide , doxorubicin , cisplatin ) ( 59 patients ) ; or arm 3 : control arm ( no maintenance treatment ) ( 87 patients ) .
	manualset3
101146	2	401251	13	NULL	NULL	0	NULL	 induction CT + RT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	237 patients who completed induction CT + RT and were classified as responders ( complete response + partial response ) were randomly assigned to arm 1 : low dose nIFN-alpha ( 91 patients ) ; arm 2 : maintenance CT , six cycles of CAP ( cyclophosphamide , doxorubicin , cisplatin ) ( 59 patients ) ; or arm 3 : control arm ( no maintenance treatment ) ( 87 patients ) .
	manualset3
101147	3	401251	13	NULL	NULL	0	NULL	responders	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	237 patients who completed induction CT + RT and were classified as responders ( complete response + partial response ) were randomly assigned to arm 1 : low dose nIFN-alpha ( 91 patients ) ; arm 2 : maintenance CT , six cycles of CAP ( cyclophosphamide , doxorubicin , cisplatin ) ( 59 patients ) ; or arm 3 : control arm ( no maintenance treatment ) ( 87 patients ) .
	manualset3
101148	4	401251	13	NULL	NULL	0	NULL	complete response + partial response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	237 patients who completed induction CT + RT and were classified as responders ( complete response + partial response ) were randomly assigned to arm 1 : low dose nIFN-alpha ( 91 patients ) ; arm 2 : maintenance CT , six cycles of CAP ( cyclophosphamide , doxorubicin , cisplatin ) ( 59 patients ) ; or arm 3 : control arm ( no maintenance treatment ) ( 87 patients ) .
	manualset3
101149	5	401251	13	NULL	NULL	0	NULL	 arm 1 : low dose nIFN-alpha	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	237 patients who completed induction CT + RT and were classified as responders ( complete response + partial response ) were randomly assigned to arm 1 : low dose nIFN-alpha ( 91 patients ) ; arm 2 : maintenance CT , six cycles of CAP ( cyclophosphamide , doxorubicin , cisplatin ) ( 59 patients ) ; or arm 3 : control arm ( no maintenance treatment ) ( 87 patients ) .
	manualset3
101150	6	401251	13	NULL	NULL	0	NULL	91 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	237 patients who completed induction CT + RT and were classified as responders ( complete response + partial response ) were randomly assigned to arm 1 : low dose nIFN-alpha ( 91 patients ) ; arm 2 : maintenance CT , six cycles of CAP ( cyclophosphamide , doxorubicin , cisplatin ) ( 59 patients ) ; or arm 3 : control arm ( no maintenance treatment ) ( 87 patients ) .
	manualset3
101151	7	401251	13	NULL	NULL	0	NULL	arm 2 : maintenance CT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	237 patients who completed induction CT + RT and were classified as responders ( complete response + partial response ) were randomly assigned to arm 1 : low dose nIFN-alpha ( 91 patients ) ; arm 2 : maintenance CT , six cycles of CAP ( cyclophosphamide , doxorubicin , cisplatin ) ( 59 patients ) ; or arm 3 : control arm ( no maintenance treatment ) ( 87 patients ) .
	manualset3
101152	8	401251	13	NULL	NULL	0	NULL	six cycles of CAP	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	237 patients who completed induction CT + RT and were classified as responders ( complete response + partial response ) were randomly assigned to arm 1 : low dose nIFN-alpha ( 91 patients ) ; arm 2 : maintenance CT , six cycles of CAP ( cyclophosphamide , doxorubicin , cisplatin ) ( 59 patients ) ; or arm 3 : control arm ( no maintenance treatment ) ( 87 patients ) .
	manualset3
101153	9	401251	13	NULL	NULL	0	NULL	 cyclophosphamide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	237 patients who completed induction CT + RT and were classified as responders ( complete response + partial response ) were randomly assigned to arm 1 : low dose nIFN-alpha ( 91 patients ) ; arm 2 : maintenance CT , six cycles of CAP ( cyclophosphamide , doxorubicin , cisplatin ) ( 59 patients ) ; or arm 3 : control arm ( no maintenance treatment ) ( 87 patients ) .
	manualset3
101154	10	401251	13	NULL	NULL	0	NULL	doxorubicin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	237 patients who completed induction CT + RT and were classified as responders ( complete response + partial response ) were randomly assigned to arm 1 : low dose nIFN-alpha ( 91 patients ) ; arm 2 : maintenance CT , six cycles of CAP ( cyclophosphamide , doxorubicin , cisplatin ) ( 59 patients ) ; or arm 3 : control arm ( no maintenance treatment ) ( 87 patients ) .
	manualset3
101155	11	401251	13	NULL	NULL	0	NULL	cisplatin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	237 patients who completed induction CT + RT and were classified as responders ( complete response + partial response ) were randomly assigned to arm 1 : low dose nIFN-alpha ( 91 patients ) ; arm 2 : maintenance CT , six cycles of CAP ( cyclophosphamide , doxorubicin , cisplatin ) ( 59 patients ) ; or arm 3 : control arm ( no maintenance treatment ) ( 87 patients ) .
	manualset3
101156	12	401251	13	NULL	NULL	0	NULL	59 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	237 patients who completed induction CT + RT and were classified as responders ( complete response + partial response ) were randomly assigned to arm 1 : low dose nIFN-alpha ( 91 patients ) ; arm 2 : maintenance CT , six cycles of CAP ( cyclophosphamide , doxorubicin , cisplatin ) ( 59 patients ) ; or arm 3 : control arm ( no maintenance treatment ) ( 87 patients ) .
	manualset3
101157	13	401251	13	NULL	NULL	NULL	NULL	arm 3 : control arm	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	237 patients who completed induction CT + RT and were classified as responders ( complete response + partial response ) were randomly assigned to arm 1 : low dose nIFN-alpha ( 91 patients ) ; arm 2 : maintenance CT , six cycles of CAP ( cyclophosphamide , doxorubicin , cisplatin ) ( 59 patients ) ; or arm 3 : control arm ( no maintenance treatment ) ( 87 patients ) .
	manualset3
101158	14	401251	13	NULL	NULL	0	NULL	no maintenance treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	237 patients who completed induction CT + RT and were classified as responders ( complete response + partial response ) were randomly assigned to arm 1 : low dose nIFN-alpha ( 91 patients ) ; arm 2 : maintenance CT , six cycles of CAP ( cyclophosphamide , doxorubicin , cisplatin ) ( 59 patients ) ; or arm 3 : control arm ( no maintenance treatment ) ( 87 patients ) .
	manualset3
101159	15	401251	13	NULL	NULL	0	NULL	 87 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	237 patients who completed induction CT + RT and were classified as responders ( complete response + partial response ) were randomly assigned to arm 1 : low dose nIFN-alpha ( 91 patients ) ; arm 2 : maintenance CT , six cycles of CAP ( cyclophosphamide , doxorubicin , cisplatin ) ( 59 patients ) ; or arm 3 : control arm ( no maintenance treatment ) ( 87 patients ) .
	manualset3
101160	1	401252	13	NULL	NULL	0	NULL	Influenza viruses 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Influenza viruses : from birds to humans .
	manualset3
101161	2	401252	13	NULL	NULL	0	NULL	birds	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Influenza viruses : from birds to humans .
	manualset3
101162	3	401252	13	NULL	NULL	0	NULL	humans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Influenza viruses : from birds to humans .
	manualset3
101163	1	401253	13	NULL	NULL	0	NULL	Information gain	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Information gain rather than error minimization is used to guide the growth of the network , which increases the utility of newly added network elements and decreases the likelihood that a premature dead end in the growth of the network will occur .
	manualset3
101164	2	401253	13	NULL	NULL	0	NULL	error minimization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Information gain rather than error minimization is used to guide the growth of the network , which increases the utility of newly added network elements and decreases the likelihood that a premature dead end in the growth of the network will occur .
	manualset3
101165	3	401253	13	NULL	NULL	0	NULL	 growth	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Information gain rather than error minimization is used to guide the growth of the network , which increases the utility of newly added network elements and decreases the likelihood that a premature dead end in the growth of the network will occur .
	manualset3
101166	4	401253	13	NULL	NULL	0	NULL	 network 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Information gain rather than error minimization is used to guide the growth of the network , which increases the utility of newly added network elements and decreases the likelihood that a premature dead end in the growth of the network will occur .
	manualset3
101167	5	401253	13	NULL	NULL	0	NULL	utility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Information gain rather than error minimization is used to guide the growth of the network , which increases the utility of newly added network elements and decreases the likelihood that a premature dead end in the growth of the network will occur .
	manualset3
101168	6	401253	13	NULL	NULL	0	NULL	network elements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Information gain rather than error minimization is used to guide the growth of the network , which increases the utility of newly added network elements and decreases the likelihood that a premature dead end in the growth of the network will occur .
	manualset3
101169	7	401253	13	NULL	NULL	0	NULL	dead end	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Information gain rather than error minimization is used to guide the growth of the network , which increases the utility of newly added network elements and decreases the likelihood that a premature dead end in the growth of the network will occur .
	manualset3
101170	8	401253	13	NULL	NULL	0	NULL	growth	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Information gain rather than error minimization is used to guide the growth of the network , which increases the utility of newly added network elements and decreases the likelihood that a premature dead end in the growth of the network will occur .
	manualset3
101171	9	401253	13	NULL	NULL	0	NULL	network 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Information gain rather than error minimization is used to guide the growth of the network , which increases the utility of newly added network elements and decreases the likelihood that a premature dead end in the growth of the network will occur .
	manualset3
101172	1	401254	13	NULL	NULL	NULL	NULL	Information	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Information in persistent firing duration was significantly greater than in spike rate , and the majority of neurons displayed more information in persistent firing , which was more likely to be observed in response to aggressive vocalizations ( 64 % ) than appeasement vocalizations ( 25 % ) , suggesting that persistent firing may relate to the behavioral context of vocalizations .
	manualset3
101173	2	401254	13	NULL	NULL	0	NULL	firing duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Information in persistent firing duration was significantly greater than in spike rate , and the majority of neurons displayed more information in persistent firing , which was more likely to be observed in response to aggressive vocalizations ( 64 % ) than appeasement vocalizations ( 25 % ) , suggesting that persistent firing may relate to the behavioral context of vocalizations .
	manualset3
101174	3	401254	13	NULL	NULL	NULL	NULL	spike rate	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Information in persistent firing duration was significantly greater than in spike rate , and the majority of neurons displayed more information in persistent firing , which was more likely to be observed in response to aggressive vocalizations ( 64 % ) than appeasement vocalizations ( 25 % ) , suggesting that persistent firing may relate to the behavioral context of vocalizations .
	manualset3
101175	4	401254	13	NULL	NULL	0	NULL	majority of neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Information in persistent firing duration was significantly greater than in spike rate , and the majority of neurons displayed more information in persistent firing , which was more likely to be observed in response to aggressive vocalizations ( 64 % ) than appeasement vocalizations ( 25 % ) , suggesting that persistent firing may relate to the behavioral context of vocalizations .
	manualset3
101176	5	401254	13	NULL	NULL	NULL	NULL	information	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Information in persistent firing duration was significantly greater than in spike rate , and the majority of neurons displayed more information in persistent firing , which was more likely to be observed in response to aggressive vocalizations ( 64 % ) than appeasement vocalizations ( 25 % ) , suggesting that persistent firing may relate to the behavioral context of vocalizations .
	manualset3
101177	6	401254	13	NULL	NULL	NULL	NULL	persistent firing	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Information in persistent firing duration was significantly greater than in spike rate , and the majority of neurons displayed more information in persistent firing , which was more likely to be observed in response to aggressive vocalizations ( 64 % ) than appeasement vocalizations ( 25 % ) , suggesting that persistent firing may relate to the behavioral context of vocalizations .
	manualset3
101178	7	401254	13	NULL	NULL	NULL	NULL	response	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Information in persistent firing duration was significantly greater than in spike rate , and the majority of neurons displayed more information in persistent firing , which was more likely to be observed in response to aggressive vocalizations ( 64 % ) than appeasement vocalizations ( 25 % ) , suggesting that persistent firing may relate to the behavioral context of vocalizations .
	manualset3
101179	8	401254	13	NULL	NULL	0	NULL	aggressive vocalizations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Information in persistent firing duration was significantly greater than in spike rate , and the majority of neurons displayed more information in persistent firing , which was more likely to be observed in response to aggressive vocalizations ( 64 % ) than appeasement vocalizations ( 25 % ) , suggesting that persistent firing may relate to the behavioral context of vocalizations .
	manualset3
101180	9	401254	13	NULL	NULL	0	NULL	 64 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Information in persistent firing duration was significantly greater than in spike rate , and the majority of neurons displayed more information in persistent firing , which was more likely to be observed in response to aggressive vocalizations ( 64 % ) than appeasement vocalizations ( 25 % ) , suggesting that persistent firing may relate to the behavioral context of vocalizations .
	manualset3
101181	10	401254	13	NULL	NULL	NULL	NULL	appeasement vocalizations	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Information in persistent firing duration was significantly greater than in spike rate , and the majority of neurons displayed more information in persistent firing , which was more likely to be observed in response to aggressive vocalizations ( 64 % ) than appeasement vocalizations ( 25 % ) , suggesting that persistent firing may relate to the behavioral context of vocalizations .
	manualset3
101182	11	401254	13	NULL	NULL	NULL	NULL	25 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Information in persistent firing duration was significantly greater than in spike rate , and the majority of neurons displayed more information in persistent firing , which was more likely to be observed in response to aggressive vocalizations ( 64 % ) than appeasement vocalizations ( 25 % ) , suggesting that persistent firing may relate to the behavioral context of vocalizations .
	manualset3
101183	12	401254	13	NULL	NULL	0	NULL	persistent firing 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Information in persistent firing duration was significantly greater than in spike rate , and the majority of neurons displayed more information in persistent firing , which was more likely to be observed in response to aggressive vocalizations ( 64 % ) than appeasement vocalizations ( 25 % ) , suggesting that persistent firing may relate to the behavioral context of vocalizations .
	manualset3
101184	13	401254	13	NULL	NULL	0	NULL	behavioral context of vocalizations 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Information in persistent firing duration was significantly greater than in spike rate , and the majority of neurons displayed more information in persistent firing , which was more likely to be observed in response to aggressive vocalizations ( 64 % ) than appeasement vocalizations ( 25 % ) , suggesting that persistent firing may relate to the behavioral context of vocalizations .
	manualset3
101185	1	401255	13	NULL	NULL	NULL	NULL	Information	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Information now available suggests an initial action of chloroquine on Golgi or smooth endoplasmic reticulum vesicles , and on granules , with alterations in their membranes leading to fusion with one another and with pinosomes .
	manualset3
101186	2	401255	13	NULL	NULL	NULL	NULL	action	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Information now available suggests an initial action of chloroquine on Golgi or smooth endoplasmic reticulum vesicles , and on granules , with alterations in their membranes leading to fusion with one another and with pinosomes .
	manualset3
101187	3	401255	13	NULL	NULL	0	NULL	chloroquine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Information now available suggests an initial action of chloroquine on Golgi or smooth endoplasmic reticulum vesicles , and on granules , with alterations in their membranes leading to fusion with one another and with pinosomes .
	manualset3
101188	4	401255	13	NULL	NULL	0	NULL	Golgi	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Information now available suggests an initial action of chloroquine on Golgi or smooth endoplasmic reticulum vesicles , and on granules , with alterations in their membranes leading to fusion with one another and with pinosomes .
	manualset3
101189	5	401255	13	NULL	NULL	0	NULL	smooth endoplasmic reticulum vesicles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Information now available suggests an initial action of chloroquine on Golgi or smooth endoplasmic reticulum vesicles , and on granules , with alterations in their membranes leading to fusion with one another and with pinosomes .
	manualset3
101190	6	401255	13	NULL	NULL	0	NULL	granules 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Information now available suggests an initial action of chloroquine on Golgi or smooth endoplasmic reticulum vesicles , and on granules , with alterations in their membranes leading to fusion with one another and with pinosomes .
	manualset3
101191	7	401255	13	NULL	NULL	0	NULL	alterations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Information now available suggests an initial action of chloroquine on Golgi or smooth endoplasmic reticulum vesicles , and on granules , with alterations in their membranes leading to fusion with one another and with pinosomes .
	manualset3
101192	8	401255	13	NULL	NULL	0	NULL	membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Information now available suggests an initial action of chloroquine on Golgi or smooth endoplasmic reticulum vesicles , and on granules , with alterations in their membranes leading to fusion with one another and with pinosomes .
	manualset3
101193	9	401255	13	NULL	NULL	0	NULL	fusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Information now available suggests an initial action of chloroquine on Golgi or smooth endoplasmic reticulum vesicles , and on granules , with alterations in their membranes leading to fusion with one another and with pinosomes .
	manualset3
101194	10	401255	13	NULL	NULL	0	NULL	pinosomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Information now available suggests an initial action of chloroquine on Golgi or smooth endoplasmic reticulum vesicles , and on granules , with alterations in their membranes leading to fusion with one another and with pinosomes .
	manualset3
101195	1	401256	13	NULL	NULL	0	NULL	Information	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Information on gastric leiomyosarcoma , such as important prognostic factors , patterns of disease recurrence , and optimal methods of treatment , are derived from limited patient experience .
	manualset3
101196	2	401256	13	NULL	NULL	0	NULL	 gastric leiomyosarcoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Information on gastric leiomyosarcoma , such as important prognostic factors , patterns of disease recurrence , and optimal methods of treatment , are derived from limited patient experience .
	manualset3
101197	3	401256	13	NULL	NULL	0	NULL	prognostic factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Information on gastric leiomyosarcoma , such as important prognostic factors , patterns of disease recurrence , and optimal methods of treatment , are derived from limited patient experience .
	manualset3
101198	4	401256	13	NULL	NULL	0	NULL	 patterns of disease recurrence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Information on gastric leiomyosarcoma , such as important prognostic factors , patterns of disease recurrence , and optimal methods of treatment , are derived from limited patient experience .
	manualset3
101199	5	401256	13	NULL	NULL	0	NULL	optimal methods 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Information on gastric leiomyosarcoma , such as important prognostic factors , patterns of disease recurrence , and optimal methods of treatment , are derived from limited patient experience .
	manualset3
101200	6	401256	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Information on gastric leiomyosarcoma , such as important prognostic factors , patterns of disease recurrence , and optimal methods of treatment , are derived from limited patient experience .
	manualset3
101201	7	401256	13	NULL	NULL	0	NULL	patient experience	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Information on gastric leiomyosarcoma , such as important prognostic factors , patterns of disease recurrence , and optimal methods of treatment , are derived from limited patient experience .
	manualset3
101202	1	401257	13	NULL	NULL	NULL	NULL	Information	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Information on the presence , structure and function of class-I helical cytokines in non-mammalian vertebrates and non-vertebrates is fragmentary .
	manualset3
101203	2	401257	13	NULL	NULL	NULL	NULL	presence	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Information on the presence , structure and function of class-I helical cytokines in non-mammalian vertebrates and non-vertebrates is fragmentary .
	manualset3
101204	3	401257	13	NULL	NULL	0	NULL	structure 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Information on the presence , structure and function of class-I helical cytokines in non-mammalian vertebrates and non-vertebrates is fragmentary .
	manualset3
101205	4	401257	13	NULL	NULL	0	NULL	function 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Information on the presence , structure and function of class-I helical cytokines in non-mammalian vertebrates and non-vertebrates is fragmentary .
	manualset3
101206	5	401257	13	NULL	NULL	0	NULL	class-I helical cytokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Information on the presence , structure and function of class-I helical cytokines in non-mammalian vertebrates and non-vertebrates is fragmentary .
	manualset3
101207	6	401257	13	NULL	NULL	0	NULL	non-mammalian vertebrates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Information on the presence , structure and function of class-I helical cytokines in non-mammalian vertebrates and non-vertebrates is fragmentary .
	manualset3
101208	7	401257	13	NULL	NULL	0	NULL	non-vertebrates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Information on the presence , structure and function of class-I helical cytokines in non-mammalian vertebrates and non-vertebrates is fragmentary .
	manualset3
101209	1	401258	13	NULL	NULL	0	NULL	Information	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Information processing during two types of EEG activity .
	manualset3
101210	2	401258	13	NULL	NULL	0	NULL	processing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Information processing during two types of EEG activity .
	manualset3
101211	3	401258	13	NULL	NULL	0	NULL	two types	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Information processing during two types of EEG activity .
	manualset3
101212	4	401258	13	NULL	NULL	0	NULL	EEG activity	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Information processing during two types of EEG activity .
	manualset3
101213	1	401259	13	NULL	NULL	0	NULL	24	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	24 cats underwent partial maxillectomies and reconstruction by TME Vascular infusion was performed immediately following sacrifice and then analyzed by radiography , light and SEM .
	manualset3
101214	2	401259	13	NULL	NULL	0	NULL	cats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	24 cats underwent partial maxillectomies and reconstruction by TME Vascular infusion was performed immediately following sacrifice and then analyzed by radiography , light and SEM .
	manualset3
101215	3	401259	13	NULL	NULL	0	NULL	partial maxillectomies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	24 cats underwent partial maxillectomies and reconstruction by TME Vascular infusion was performed immediately following sacrifice and then analyzed by radiography , light and SEM .
	manualset3
101216	4	401259	13	NULL	NULL	0	NULL	reconstruction	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	24 cats underwent partial maxillectomies and reconstruction by TME Vascular infusion was performed immediately following sacrifice and then analyzed by radiography , light and SEM .
	manualset3
101217	5	401259	13	NULL	NULL	0	NULL	 TME Vascular infusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	24 cats underwent partial maxillectomies and reconstruction by TME Vascular infusion was performed immediately following sacrifice and then analyzed by radiography , light and SEM .
	manualset3
101218	6	401259	13	NULL	NULL	0	NULL	sacrifice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	24 cats underwent partial maxillectomies and reconstruction by TME Vascular infusion was performed immediately following sacrifice and then analyzed by radiography , light and SEM .
	manualset3
101219	7	401259	13	NULL	NULL	0	NULL	radiography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	24 cats underwent partial maxillectomies and reconstruction by TME Vascular infusion was performed immediately following sacrifice and then analyzed by radiography , light and SEM .
	manualset3
101220	8	401259	13	NULL	NULL	0	NULL	light	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	24 cats underwent partial maxillectomies and reconstruction by TME Vascular infusion was performed immediately following sacrifice and then analyzed by radiography , light and SEM .
	manualset3
101221	9	401259	13	NULL	NULL	0	NULL	 SEM	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	24 cats underwent partial maxillectomies and reconstruction by TME Vascular infusion was performed immediately following sacrifice and then analyzed by radiography , light and SEM .
	manualset3
101222	1	401260	13	NULL	NULL	0	NULL	Information technology 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Information technology and today 's health care management .
	manualset3
101223	2	401260	13	NULL	NULL	0	NULL	today 's	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Information technology and today 's health care management .
	manualset3
101224	3	401260	13	NULL	NULL	0	NULL	health care management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Information technology and today 's health care management .
	manualset3
101225	1	401261	13	NULL	NULL	0	NULL	adherence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Informed adherence : the need for shared medical decision making .
	manualset3
101226	2	401261	13	NULL	NULL	0	NULL	need	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Informed adherence : the need for shared medical decision making .
	manualset3
101227	3	401261	13	NULL	NULL	0	NULL	medical decision	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Informed adherence : the need for shared medical decision making .
	manualset3
101228	1	401262	13	NULL	NULL	0	NULL	Infusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusion of imidazole ( 50-75 microgram/ml ) through the lung or spleen specifically inhibits thromboxane A2 production and diverts the pathway to the prostaglandins , mainly prostaglandin F2alpha .
	manualset3
101229	2	401262	13	NULL	NULL	0	NULL	 imidazole	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusion of imidazole ( 50-75 microgram/ml ) through the lung or spleen specifically inhibits thromboxane A2 production and diverts the pathway to the prostaglandins , mainly prostaglandin F2alpha .
	manualset3
101230	3	401262	13	NULL	NULL	0	NULL	50-75 microgram/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusion of imidazole ( 50-75 microgram/ml ) through the lung or spleen specifically inhibits thromboxane A2 production and diverts the pathway to the prostaglandins , mainly prostaglandin F2alpha .
	manualset3
101231	4	401262	13	NULL	NULL	0	NULL	lung	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusion of imidazole ( 50-75 microgram/ml ) through the lung or spleen specifically inhibits thromboxane A2 production and diverts the pathway to the prostaglandins , mainly prostaglandin F2alpha .
	manualset3
101232	5	401262	13	NULL	NULL	0	NULL	 spleen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusion of imidazole ( 50-75 microgram/ml ) through the lung or spleen specifically inhibits thromboxane A2 production and diverts the pathway to the prostaglandins , mainly prostaglandin F2alpha .
	manualset3
101233	6	401262	13	NULL	NULL	0	NULL	thromboxane A2 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusion of imidazole ( 50-75 microgram/ml ) through the lung or spleen specifically inhibits thromboxane A2 production and diverts the pathway to the prostaglandins , mainly prostaglandin F2alpha .
	manualset3
101234	7	401262	13	NULL	NULL	0	NULL	production 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusion of imidazole ( 50-75 microgram/ml ) through the lung or spleen specifically inhibits thromboxane A2 production and diverts the pathway to the prostaglandins , mainly prostaglandin F2alpha .
	manualset3
101235	8	401262	13	NULL	NULL	0	NULL	pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusion of imidazole ( 50-75 microgram/ml ) through the lung or spleen specifically inhibits thromboxane A2 production and diverts the pathway to the prostaglandins , mainly prostaglandin F2alpha .
	manualset3
101236	9	401262	13	NULL	NULL	0	NULL	prostaglandins 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusion of imidazole ( 50-75 microgram/ml ) through the lung or spleen specifically inhibits thromboxane A2 production and diverts the pathway to the prostaglandins , mainly prostaglandin F2alpha .
	manualset3
101237	10	401262	13	NULL	NULL	0	NULL	prostaglandin F2alpha	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusion of imidazole ( 50-75 microgram/ml ) through the lung or spleen specifically inhibits thromboxane A2 production and diverts the pathway to the prostaglandins , mainly prostaglandin F2alpha .
	manualset3
101238	1	401263	13	NULL	NULL	0	NULL	Infusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusion of pentylenetetrazol ( PTZ ) induced epileptic discharges on the EEG and caused an increase in blood pressure .
	manualset3
101239	2	401263	13	NULL	NULL	0	NULL	pentylenetetrazol ( PTZ ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusion of pentylenetetrazol ( PTZ ) induced epileptic discharges on the EEG and caused an increase in blood pressure .
	manualset3
101240	3	401263	13	NULL	NULL	0	NULL	epileptic discharges	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusion of pentylenetetrazol ( PTZ ) induced epileptic discharges on the EEG and caused an increase in blood pressure .
	manualset3
101241	4	401263	13	NULL	NULL	0	NULL	EEG	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusion of pentylenetetrazol ( PTZ ) induced epileptic discharges on the EEG and caused an increase in blood pressure .
	manualset3
101242	5	401263	13	NULL	NULL	0	NULL	increase in blood pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusion of pentylenetetrazol ( PTZ ) induced epileptic discharges on the EEG and caused an increase in blood pressure .
	manualset3
101243	1	401264	13	NULL	NULL	0	NULL	Infusion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusion of soy and casein protein meals affects interorgan amino acid metabolism and urea kinetics differently in pigs .
	manualset3
101244	2	401264	13	NULL	NULL	0	NULL	soy meals 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusion of soy and casein protein meals affects interorgan amino acid metabolism and urea kinetics differently in pigs .
	manualset3
101245	3	401264	13	NULL	NULL	0	NULL	casein protein meals	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusion of soy and casein protein meals affects interorgan amino acid metabolism and urea kinetics differently in pigs .
	manualset3
101246	4	401264	13	NULL	NULL	0	NULL	interorgan amino acid metabolism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusion of soy and casein protein meals affects interorgan amino acid metabolism and urea kinetics differently in pigs .
	manualset3
101247	5	401264	13	NULL	NULL	0	NULL	urea kinetics	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusion of soy and casein protein meals affects interorgan amino acid metabolism and urea kinetics differently in pigs .
	manualset3
101248	6	401264	13	NULL	NULL	0	NULL	 pigs 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusion of soy and casein protein meals affects interorgan amino acid metabolism and urea kinetics differently in pigs .
	manualset3
101249	1	401265	13	NULL	NULL	0	NULL	Infusion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusion of up to 100 ( PGF ) mcq/min of PGF2alpha resulted in regular uterine contractions within the first 2 hours .
	manualset3
101250	2	401265	13	NULL	NULL	0	NULL	100 ( PGF ) mcq/min	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusion of up to 100 ( PGF ) mcq/min of PGF2alpha resulted in regular uterine contractions within the first 2 hours .
	manualset3
101251	3	401265	13	NULL	NULL	0	NULL	PGF2alpha 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusion of up to 100 ( PGF ) mcq/min of PGF2alpha resulted in regular uterine contractions within the first 2 hours .
	manualset3
101252	4	401265	13	NULL	NULL	0	NULL	uterine contractions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusion of up to 100 ( PGF ) mcq/min of PGF2alpha resulted in regular uterine contractions within the first 2 hours .
	manualset3
101253	5	401265	13	NULL	NULL	0	NULL	first 2 hours	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusion of up to 100 ( PGF ) mcq/min of PGF2alpha resulted in regular uterine contractions within the first 2 hours .
	manualset3
101254	1	401266	13	NULL	NULL	0	NULL	Infusions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusions were discontinued at the end of the occlusion and data were analyzed for the following 8 h. A transient , secondary fall in carotid artery blood flow and laser Doppler flow was seen from approximately 1-4 h after occlusion ( P & lt ; 0.001 ) , with no significant differences between vehicle and DPCPX .
	manualset3
101255	2	401266	13	NULL	NULL	0	NULL	end	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusions were discontinued at the end of the occlusion and data were analyzed for the following 8 h. A transient , secondary fall in carotid artery blood flow and laser Doppler flow was seen from approximately 1-4 h after occlusion ( P & lt ; 0.001 ) , with no significant differences between vehicle and DPCPX .
	manualset3
101256	3	401266	13	NULL	NULL	0	NULL	occlusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusions were discontinued at the end of the occlusion and data were analyzed for the following 8 h. A transient , secondary fall in carotid artery blood flow and laser Doppler flow was seen from approximately 1-4 h after occlusion ( P & lt ; 0.001 ) , with no significant differences between vehicle and DPCPX .
	manualset3
101257	4	401266	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusions were discontinued at the end of the occlusion and data were analyzed for the following 8 h. A transient , secondary fall in carotid artery blood flow and laser Doppler flow was seen from approximately 1-4 h after occlusion ( P & lt ; 0.001 ) , with no significant differences between vehicle and DPCPX .
	manualset3
101258	5	401266	13	NULL	NULL	0	NULL	8 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusions were discontinued at the end of the occlusion and data were analyzed for the following 8 h. A transient , secondary fall in carotid artery blood flow and laser Doppler flow was seen from approximately 1-4 h after occlusion ( P & lt ; 0.001 ) , with no significant differences between vehicle and DPCPX .
	manualset3
101259	6	401266	13	NULL	NULL	0	NULL	carotid artery blood flow	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusions were discontinued at the end of the occlusion and data were analyzed for the following 8 h. A transient , secondary fall in carotid artery blood flow and laser Doppler flow was seen from approximately 1-4 h after occlusion ( P & lt ; 0.001 ) , with no significant differences between vehicle and DPCPX .
	manualset3
101260	7	401266	13	NULL	NULL	0	NULL	laser Doppler flow 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusions were discontinued at the end of the occlusion and data were analyzed for the following 8 h. A transient , secondary fall in carotid artery blood flow and laser Doppler flow was seen from approximately 1-4 h after occlusion ( P & lt ; 0.001 ) , with no significant differences between vehicle and DPCPX .
	manualset3
101261	8	401266	13	NULL	NULL	0	NULL	1-4 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusions were discontinued at the end of the occlusion and data were analyzed for the following 8 h. A transient , secondary fall in carotid artery blood flow and laser Doppler flow was seen from approximately 1-4 h after occlusion ( P & lt ; 0.001 ) , with no significant differences between vehicle and DPCPX .
	manualset3
101262	9	401266	13	NULL	NULL	0	NULL	occlusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusions were discontinued at the end of the occlusion and data were analyzed for the following 8 h. A transient , secondary fall in carotid artery blood flow and laser Doppler flow was seen from approximately 1-4 h after occlusion ( P & lt ; 0.001 ) , with no significant differences between vehicle and DPCPX .
	manualset3
101263	10	401266	13	NULL	NULL	0	NULL	P & lt ; 0.001 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusions were discontinued at the end of the occlusion and data were analyzed for the following 8 h. A transient , secondary fall in carotid artery blood flow and laser Doppler flow was seen from approximately 1-4 h after occlusion ( P & lt ; 0.001 ) , with no significant differences between vehicle and DPCPX .
	manualset3
101264	11	401266	13	NULL	NULL	0	NULL	differences 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusions were discontinued at the end of the occlusion and data were analyzed for the following 8 h. A transient , secondary fall in carotid artery blood flow and laser Doppler flow was seen from approximately 1-4 h after occlusion ( P & lt ; 0.001 ) , with no significant differences between vehicle and DPCPX .
	manualset3
101265	12	401266	13	NULL	NULL	0	NULL	vehicle	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusions were discontinued at the end of the occlusion and data were analyzed for the following 8 h. A transient , secondary fall in carotid artery blood flow and laser Doppler flow was seen from approximately 1-4 h after occlusion ( P & lt ; 0.001 ) , with no significant differences between vehicle and DPCPX .
	manualset3
101266	13	401266	13	NULL	NULL	0	NULL	DPCPX	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Infusions were discontinued at the end of the occlusion and data were analyzed for the following 8 h. A transient , secondary fall in carotid artery blood flow and laser Doppler flow was seen from approximately 1-4 h after occlusion ( P & lt ; 0.001 ) , with no significant differences between vehicle and DPCPX .
	manualset3
101267	1	401267	13	NULL	NULL	0	NULL	Ingestion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ingestion of highly palatable diets ( HPDs ) , rich in sucrose and fat , has been shown to lead to obesity and alterations in cardiovascular function in animal models .
	manualset3
101268	2	401267	13	NULL	NULL	0	NULL	highly palatable diets ( HPDs ) 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Ingestion of highly palatable diets ( HPDs ) , rich in sucrose and fat , has been shown to lead to obesity and alterations in cardiovascular function in animal models .
	manualset3
101269	3	401267	13	NULL	NULL	NULL	NULL	sucrose	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ingestion of highly palatable diets ( HPDs ) , rich in sucrose and fat , has been shown to lead to obesity and alterations in cardiovascular function in animal models .
	manualset3
101270	4	401267	13	NULL	NULL	0	NULL	fat	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ingestion of highly palatable diets ( HPDs ) , rich in sucrose and fat , has been shown to lead to obesity and alterations in cardiovascular function in animal models .
	manualset3
101271	5	401267	13	NULL	NULL	0	NULL	obesity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ingestion of highly palatable diets ( HPDs ) , rich in sucrose and fat , has been shown to lead to obesity and alterations in cardiovascular function in animal models .
	manualset3
101272	6	401267	13	NULL	NULL	0	NULL	alterations 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ingestion of highly palatable diets ( HPDs ) , rich in sucrose and fat , has been shown to lead to obesity and alterations in cardiovascular function in animal models .
	manualset3
101273	7	401267	13	NULL	NULL	0	NULL	cardiovascular function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ingestion of highly palatable diets ( HPDs ) , rich in sucrose and fat , has been shown to lead to obesity and alterations in cardiovascular function in animal models .
	manualset3
101274	8	401267	13	NULL	NULL	0	NULL	animal models	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ingestion of highly palatable diets ( HPDs ) , rich in sucrose and fat , has been shown to lead to obesity and alterations in cardiovascular function in animal models .
	manualset3
101275	1	401268	13	NULL	NULL	0	NULL	Ingrowth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ingrowth of this hypervascularized , pyogenic granuloma-like tissue is presumably due to the presence of excessive growth factors , reflecting an exaggerated pathophysiological reaction within the framework of organization of the necrotic epiphyses .
	manualset3
101276	2	401268	13	NULL	NULL	0	NULL	pyogenic granuloma-like tissue 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Ingrowth of this hypervascularized , pyogenic granuloma-like tissue is presumably due to the presence of excessive growth factors , reflecting an exaggerated pathophysiological reaction within the framework of organization of the necrotic epiphyses .
	manualset3
101277	3	401268	13	NULL	NULL	0	NULL	presence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ingrowth of this hypervascularized , pyogenic granuloma-like tissue is presumably due to the presence of excessive growth factors , reflecting an exaggerated pathophysiological reaction within the framework of organization of the necrotic epiphyses .
	manualset3
101278	4	401268	13	NULL	NULL	0	NULL	growth factors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ingrowth of this hypervascularized , pyogenic granuloma-like tissue is presumably due to the presence of excessive growth factors , reflecting an exaggerated pathophysiological reaction within the framework of organization of the necrotic epiphyses .
	manualset3
101279	5	401268	13	NULL	NULL	0	NULL	pathophysiological reaction 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ingrowth of this hypervascularized , pyogenic granuloma-like tissue is presumably due to the presence of excessive growth factors , reflecting an exaggerated pathophysiological reaction within the framework of organization of the necrotic epiphyses .
	manualset3
101280	6	401268	13	NULL	NULL	0	NULL	framework of organization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ingrowth of this hypervascularized , pyogenic granuloma-like tissue is presumably due to the presence of excessive growth factors , reflecting an exaggerated pathophysiological reaction within the framework of organization of the necrotic epiphyses .
	manualset3
101281	7	401268	13	NULL	NULL	0	NULL	necrotic epiphyses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ingrowth of this hypervascularized , pyogenic granuloma-like tissue is presumably due to the presence of excessive growth factors , reflecting an exaggerated pathophysiological reaction within the framework of organization of the necrotic epiphyses .
	manualset3
101282	1	401269	13	NULL	NULL	0	NULL	allergic bronchial response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhaled , they reduce the early allergic bronchial response , even when ingested they aggravate the bronchial response to histamine , all the more so as their effect on the central nervous system is greater .
	manualset3
101283	2	401269	13	NULL	NULL	0	NULL	bronchial response 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhaled , they reduce the early allergic bronchial response , even when ingested they aggravate the bronchial response to histamine , all the more so as their effect on the central nervous system is greater .
	manualset3
101284	3	401269	13	NULL	NULL	0	NULL	histamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhaled , they reduce the early allergic bronchial response , even when ingested they aggravate the bronchial response to histamine , all the more so as their effect on the central nervous system is greater .
	manualset3
101285	4	401269	13	NULL	NULL	0	NULL	effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhaled , they reduce the early allergic bronchial response , even when ingested they aggravate the bronchial response to histamine , all the more so as their effect on the central nervous system is greater .
	manualset3
101286	5	401269	13	NULL	NULL	NULL	NULL	central nervous system	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Inhaled , they reduce the early allergic bronchial response , even when ingested they aggravate the bronchial response to histamine , all the more so as their effect on the central nervous system is greater .
	manualset3
101287	1	401270	13	NULL	NULL	0	NULL	corticosteroids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhaled corticosteroids are considered to be the therapy of choice in the treatment of asthma and allergic rhinitis .
	manualset3
101288	2	401270	13	NULL	NULL	0	NULL	therapy of choice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhaled corticosteroids are considered to be the therapy of choice in the treatment of asthma and allergic rhinitis .
	manualset3
101289	3	401270	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhaled corticosteroids are considered to be the therapy of choice in the treatment of asthma and allergic rhinitis .
	manualset3
101290	4	401270	13	NULL	NULL	0	NULL	asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhaled corticosteroids are considered to be the therapy of choice in the treatment of asthma and allergic rhinitis .
	manualset3
101291	5	401270	13	NULL	NULL	NULL	NULL	allergic rhinitis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Inhaled corticosteroids are considered to be the therapy of choice in the treatment of asthma and allergic rhinitis .
	manualset3
101292	1	401271	13	NULL	NULL	0	NULL	salmeterol 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhaled salmeterol : a review of its efficacy in chronic obstructive pulmonary disease .
	manualset3
101293	2	401271	13	NULL	NULL	0	NULL	review	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhaled salmeterol : a review of its efficacy in chronic obstructive pulmonary disease .
	manualset3
101294	3	401271	13	NULL	NULL	0	NULL	efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhaled salmeterol : a review of its efficacy in chronic obstructive pulmonary disease .
	manualset3
101295	4	401271	13	NULL	NULL	0	NULL	chronic obstructive pulmonary disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhaled salmeterol : a review of its efficacy in chronic obstructive pulmonary disease .
	manualset3
101296	1	401272	13	NULL	NULL	0	NULL	translocations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inherited translocations in two families ( t ( 14q + ; 10q - ) and t ( 13q - ; 21q + ) ) .
	manualset3
101297	2	401272	13	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Inherited translocations in two families ( t ( 14q + ; 10q - ) and t ( 13q - ; 21q + ) ) .
	manualset3
101298	3	401272	13	NULL	NULL	0	NULL	families	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Inherited translocations in two families ( t ( 14q + ; 10q - ) and t ( 13q - ; 21q + ) ) .
	manualset3
101299	4	401272	13	NULL	NULL	0	NULL	 ( t ( 14q + ; 10q - )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Inherited translocations in two families ( t ( 14q + ; 10q - ) and t ( 13q - ; 21q + ) ) .
	manualset3
101300	5	401272	13	NULL	NULL	0	NULL	 t ( 13q - ; 21q + ) ) 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Inherited translocations in two families ( t ( 14q + ; 10q - ) and t ( 13q - ; 21q + ) ) .
	manualset3
101301	1	401273	13	NULL	NULL	NULL	NULL	Inhibition	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Inhibition by alpha , beta-methylene-ATP , which activates ligand-gated P2X receptors , was abolished by zero Ca2 + , whereas inhibition by UTP , which activates P2Y2 receptors coupled to Gq/11 and Gi3 , was not affected by zero Ca2 + but was abolished by pertussis toxin ( PTX ) .
	manualset3
101302	2	401273	13	NULL	NULL	0	NULL	beta-methylene-ATP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition by alpha , beta-methylene-ATP , which activates ligand-gated P2X receptors , was abolished by zero Ca2 + , whereas inhibition by UTP , which activates P2Y2 receptors coupled to Gq/11 and Gi3 , was not affected by zero Ca2 + but was abolished by pertussis toxin ( PTX ) .
	manualset3
101303	3	401273	13	NULL	NULL	0	NULL	 ligand-gated P2X receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition by alpha , beta-methylene-ATP , which activates ligand-gated P2X receptors , was abolished by zero Ca2 + , whereas inhibition by UTP , which activates P2Y2 receptors coupled to Gq/11 and Gi3 , was not affected by zero Ca2 + but was abolished by pertussis toxin ( PTX ) .
	manualset3
101304	4	401273	13	NULL	NULL	0	NULL	zero Ca2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition by alpha , beta-methylene-ATP , which activates ligand-gated P2X receptors , was abolished by zero Ca2 + , whereas inhibition by UTP , which activates P2Y2 receptors coupled to Gq/11 and Gi3 , was not affected by zero Ca2 + but was abolished by pertussis toxin ( PTX ) .
	manualset3
101305	5	401273	13	NULL	NULL	NULL	NULL	inhibition	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Inhibition by alpha , beta-methylene-ATP , which activates ligand-gated P2X receptors , was abolished by zero Ca2 + , whereas inhibition by UTP , which activates P2Y2 receptors coupled to Gq/11 and Gi3 , was not affected by zero Ca2 + but was abolished by pertussis toxin ( PTX ) .
	manualset3
101306	6	401273	13	NULL	NULL	0	NULL	UTP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition by alpha , beta-methylene-ATP , which activates ligand-gated P2X receptors , was abolished by zero Ca2 + , whereas inhibition by UTP , which activates P2Y2 receptors coupled to Gq/11 and Gi3 , was not affected by zero Ca2 + but was abolished by pertussis toxin ( PTX ) .
	manualset3
101307	7	401273	13	NULL	NULL	0	NULL	P2Y2 receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition by alpha , beta-methylene-ATP , which activates ligand-gated P2X receptors , was abolished by zero Ca2 + , whereas inhibition by UTP , which activates P2Y2 receptors coupled to Gq/11 and Gi3 , was not affected by zero Ca2 + but was abolished by pertussis toxin ( PTX ) .
	manualset3
101308	8	401273	13	NULL	NULL	0	NULL	Gq/11	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition by alpha , beta-methylene-ATP , which activates ligand-gated P2X receptors , was abolished by zero Ca2 + , whereas inhibition by UTP , which activates P2Y2 receptors coupled to Gq/11 and Gi3 , was not affected by zero Ca2 + but was abolished by pertussis toxin ( PTX ) .
	manualset3
101309	9	401273	13	NULL	NULL	0	NULL	Gi3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition by alpha , beta-methylene-ATP , which activates ligand-gated P2X receptors , was abolished by zero Ca2 + , whereas inhibition by UTP , which activates P2Y2 receptors coupled to Gq/11 and Gi3 , was not affected by zero Ca2 + but was abolished by pertussis toxin ( PTX ) .
	manualset3
101310	10	401273	13	NULL	NULL	0	NULL	 zero Ca2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition by alpha , beta-methylene-ATP , which activates ligand-gated P2X receptors , was abolished by zero Ca2 + , whereas inhibition by UTP , which activates P2Y2 receptors coupled to Gq/11 and Gi3 , was not affected by zero Ca2 + but was abolished by pertussis toxin ( PTX ) .
	manualset3
101311	11	401273	13	NULL	NULL	0	NULL	pertussis toxin ( PTX )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition by alpha , beta-methylene-ATP , which activates ligand-gated P2X receptors , was abolished by zero Ca2 + , whereas inhibition by UTP , which activates P2Y2 receptors coupled to Gq/11 and Gi3 , was not affected by zero Ca2 + but was abolished by pertussis toxin ( PTX ) .
	manualset3
101312	1	401274	13	NULL	NULL	0	NULL	Inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition by nicotinamide of a homologous PCA reaction and antigen-induced histamine release from isolated rat peritoneal mast cells .
	manualset3
101313	2	401274	13	NULL	NULL	0	NULL	nicotinamide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition by nicotinamide of a homologous PCA reaction and antigen-induced histamine release from isolated rat peritoneal mast cells .
	manualset3
101314	3	401274	13	NULL	NULL	0	NULL	homologous PCA reaction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition by nicotinamide of a homologous PCA reaction and antigen-induced histamine release from isolated rat peritoneal mast cells .
	manualset3
101315	4	401274	13	NULL	NULL	0	NULL	antigen-induced histamine release	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition by nicotinamide of a homologous PCA reaction and antigen-induced histamine release from isolated rat peritoneal mast cells .
	manualset3
101316	5	401274	13	NULL	NULL	0	NULL	rat peritoneal mast cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition by nicotinamide of a homologous PCA reaction and antigen-induced histamine release from isolated rat peritoneal mast cells .
	manualset3
101317	1	401275	13	NULL	NULL	0	NULL	26	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	26 observers assessed the strength , taste , and taster 's enjoyment of the drink from video clips of the tasters .
	manualset3
101318	2	401275	13	NULL	NULL	0	NULL	 observers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	26 observers assessed the strength , taste , and taster 's enjoyment of the drink from video clips of the tasters .
	manualset3
101319	3	401275	13	NULL	NULL	0	NULL	strength	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	26 observers assessed the strength , taste , and taster 's enjoyment of the drink from video clips of the tasters .
	manualset3
101320	4	401275	13	NULL	NULL	0	NULL	taste	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	26 observers assessed the strength , taste , and taster 's enjoyment of the drink from video clips of the tasters .
	manualset3
101321	5	401275	13	NULL	NULL	0	NULL	taster 's enjoyment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	26 observers assessed the strength , taste , and taster 's enjoyment of the drink from video clips of the tasters .
	manualset3
101322	6	401275	13	NULL	NULL	0	NULL	drink	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	26 observers assessed the strength , taste , and taster 's enjoyment of the drink from video clips of the tasters .
	manualset3
101323	7	401275	13	NULL	NULL	0	NULL	video clips	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	26 observers assessed the strength , taste , and taster 's enjoyment of the drink from video clips of the tasters .
	manualset3
101324	8	401275	13	NULL	NULL	0	NULL	tasters	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	26 observers assessed the strength , taste , and taster 's enjoyment of the drink from video clips of the tasters .
	manualset3
101325	1	401276	13	NULL	NULL	NULL	NULL	Inhibition	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Inhibition of ( 3H ) thymidine incorporation by Mycoplasma arginini-infected cells due to enzymatic cleavage of the nucleoside .
	manualset3
101326	2	401276	13	NULL	NULL	0	NULL	( 3H ) thymidine incorporation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of ( 3H ) thymidine incorporation by Mycoplasma arginini-infected cells due to enzymatic cleavage of the nucleoside .
	manualset3
101327	3	401276	13	NULL	NULL	0	NULL	Mycoplasma arginini-infected cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of ( 3H ) thymidine incorporation by Mycoplasma arginini-infected cells due to enzymatic cleavage of the nucleoside .
	manualset3
101328	4	401276	13	NULL	NULL	0	NULL	enzymatic cleavage 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of ( 3H ) thymidine incorporation by Mycoplasma arginini-infected cells due to enzymatic cleavage of the nucleoside .
	manualset3
101329	5	401276	13	NULL	NULL	0	NULL	nucleoside 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of ( 3H ) thymidine incorporation by Mycoplasma arginini-infected cells due to enzymatic cleavage of the nucleoside .
	manualset3
101330	1	401277	13	NULL	NULL	NULL	NULL	Inhibition	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Inhibition of 5-HT synthesis by PCPA failed , however , to prevent lithium-induced CTA .
	manualset3
101331	2	401277	13	NULL	NULL	0	NULL	5-HT synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of 5-HT synthesis by PCPA failed , however , to prevent lithium-induced CTA .
	manualset3
101332	3	401277	13	NULL	NULL	0	NULL	PCPA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of 5-HT synthesis by PCPA failed , however , to prevent lithium-induced CTA .
	manualset3
101333	4	401277	13	NULL	NULL	0	NULL	lithium-induced CTA	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of 5-HT synthesis by PCPA failed , however , to prevent lithium-induced CTA .
	manualset3
101334	1	401278	13	NULL	NULL	0	NULL	Inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of EDTA of growth of Lactobacillus casei in the folate microbiological assay and its reversal by added manganese or iron .
	manualset3
101335	2	401278	13	NULL	NULL	0	NULL	 EDTA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of EDTA of growth of Lactobacillus casei in the folate microbiological assay and its reversal by added manganese or iron .
	manualset3
101336	3	401278	13	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of EDTA of growth of Lactobacillus casei in the folate microbiological assay and its reversal by added manganese or iron .
	manualset3
101337	4	401278	13	NULL	NULL	0	NULL	Lactobacillus casei	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of EDTA of growth of Lactobacillus casei in the folate microbiological assay and its reversal by added manganese or iron .
	manualset3
101338	5	401278	13	NULL	NULL	0	NULL	folate microbiological assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of EDTA of growth of Lactobacillus casei in the folate microbiological assay and its reversal by added manganese or iron .
	manualset3
101339	6	401278	13	NULL	NULL	0	NULL	reversal 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of EDTA of growth of Lactobacillus casei in the folate microbiological assay and its reversal by added manganese or iron .
	manualset3
101340	7	401278	13	NULL	NULL	0	NULL	manganese	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of EDTA of growth of Lactobacillus casei in the folate microbiological assay and its reversal by added manganese or iron .
	manualset3
101341	8	401278	13	NULL	NULL	0	NULL	iron	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of EDTA of growth of Lactobacillus casei in the folate microbiological assay and its reversal by added manganese or iron .
	manualset3
101342	1	401279	13	NULL	NULL	0	NULL	Inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of Ehrlich ascites cell anion transport by 1-isothiocyanate-4-benzenesulfonic acid .
	manualset3
101343	2	401279	13	NULL	NULL	0	NULL	Ehrlich ascites cell anion transport	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of Ehrlich ascites cell anion transport by 1-isothiocyanate-4-benzenesulfonic acid .
	manualset3
101344	3	401279	13	NULL	NULL	0	NULL	1-isothiocyanate-4-benzenesulfonic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of Ehrlich ascites cell anion transport by 1-isothiocyanate-4-benzenesulfonic acid .
	manualset3
101345	1	401280	13	NULL	NULL	NULL	NULL	Inhibition	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Inhibition of GRKs by using heparin or GRK2-mutant mice did not block desensitization or alter the rate of recovery from desensitization .
	manualset3
101346	2	401280	13	NULL	NULL	0	NULL	GRKs 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of GRKs by using heparin or GRK2-mutant mice did not block desensitization or alter the rate of recovery from desensitization .
	manualset3
101347	3	401280	13	NULL	NULL	0	NULL	heparin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of GRKs by using heparin or GRK2-mutant mice did not block desensitization or alter the rate of recovery from desensitization .
	manualset3
101348	4	401280	13	NULL	NULL	0	NULL	GRK2-mutant mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of GRKs by using heparin or GRK2-mutant mice did not block desensitization or alter the rate of recovery from desensitization .
	manualset3
101349	5	401280	13	NULL	NULL	0	NULL	desensitization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of GRKs by using heparin or GRK2-mutant mice did not block desensitization or alter the rate of recovery from desensitization .
	manualset3
101350	6	401280	13	NULL	NULL	0	NULL	rate of recovery 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of GRKs by using heparin or GRK2-mutant mice did not block desensitization or alter the rate of recovery from desensitization .
	manualset3
101351	7	401280	13	NULL	NULL	0	NULL	desensitization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of GRKs by using heparin or GRK2-mutant mice did not block desensitization or alter the rate of recovery from desensitization .
	manualset3
101352	1	401281	13	NULL	NULL	NULL	NULL	Inhibition 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Inhibition of Influenza A Virus ( H1N1 ) Fusion by Benzenesulfonamide Derivatives Targeting Viral Hemagglutinin .
	manualset3
101353	2	401281	13	NULL	NULL	0	NULL	 Influenza A Virus ( H1N1 ) Fusion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of Influenza A Virus ( H1N1 ) Fusion by Benzenesulfonamide Derivatives Targeting Viral Hemagglutinin .
	manualset3
101354	3	401281	13	NULL	NULL	0	NULL	Benzenesulfonamide Derivatives	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of Influenza A Virus ( H1N1 ) Fusion by Benzenesulfonamide Derivatives Targeting Viral Hemagglutinin .
	manualset3
101356	5	401281	13	NULL	NULL	0	NULL	Viral Hemagglutinin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of Influenza A Virus ( H1N1 ) Fusion by Benzenesulfonamide Derivatives Targeting Viral Hemagglutinin .
	manualset3
101357	1	401282	13	NULL	NULL	0	NULL	Inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of Jv by ANF in rat proximal straight tubules requires angiotensin .
	manualset3
101358	2	401282	13	NULL	NULL	0	NULL	Jv	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of Jv by ANF in rat proximal straight tubules requires angiotensin .
	manualset3
101359	3	401282	13	NULL	NULL	0	NULL	ANF 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of Jv by ANF in rat proximal straight tubules requires angiotensin .
	manualset3
101360	4	401282	13	NULL	NULL	0	NULL	rat proximal straight tubules	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of Jv by ANF in rat proximal straight tubules requires angiotensin .
	manualset3
101361	5	401282	13	NULL	NULL	0	NULL	angiotensin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of Jv by ANF in rat proximal straight tubules requires angiotensin .
	manualset3
101362	1	401283	13	NULL	NULL	0	NULL	Inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of PP2A activity by treatment with okadaic acid or PP2A silencing with small interfering RNA not only enhanced NF-kappaB transactivation but also prevented the increased susceptibility of IEC-TRPC1 cells to apoptosis induced by treatment with tumor necrosis factor-alpha ( TNF-alpha ) / cycloheximide ( CHX ) .
	manualset3
101363	2	401283	13	NULL	NULL	0	NULL	PP2A activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of PP2A activity by treatment with okadaic acid or PP2A silencing with small interfering RNA not only enhanced NF-kappaB transactivation but also prevented the increased susceptibility of IEC-TRPC1 cells to apoptosis induced by treatment with tumor necrosis factor-alpha ( TNF-alpha ) / cycloheximide ( CHX ) .
	manualset3
101364	3	401283	13	NULL	NULL	0	NULL	treatment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of PP2A activity by treatment with okadaic acid or PP2A silencing with small interfering RNA not only enhanced NF-kappaB transactivation but also prevented the increased susceptibility of IEC-TRPC1 cells to apoptosis induced by treatment with tumor necrosis factor-alpha ( TNF-alpha ) / cycloheximide ( CHX ) .
	manualset3
101365	4	401283	13	NULL	NULL	0	NULL	okadaic acid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of PP2A activity by treatment with okadaic acid or PP2A silencing with small interfering RNA not only enhanced NF-kappaB transactivation but also prevented the increased susceptibility of IEC-TRPC1 cells to apoptosis induced by treatment with tumor necrosis factor-alpha ( TNF-alpha ) / cycloheximide ( CHX ) .
	manualset3
101366	5	401283	13	NULL	NULL	NULL	NULL	 PP2A silencing	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Inhibition of PP2A activity by treatment with okadaic acid or PP2A silencing with small interfering RNA not only enhanced NF-kappaB transactivation but also prevented the increased susceptibility of IEC-TRPC1 cells to apoptosis induced by treatment with tumor necrosis factor-alpha ( TNF-alpha ) / cycloheximide ( CHX ) .
	manualset3
101367	6	401283	13	NULL	NULL	0	NULL	small interfering RNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of PP2A activity by treatment with okadaic acid or PP2A silencing with small interfering RNA not only enhanced NF-kappaB transactivation but also prevented the increased susceptibility of IEC-TRPC1 cells to apoptosis induced by treatment with tumor necrosis factor-alpha ( TNF-alpha ) / cycloheximide ( CHX ) .
	manualset3
101368	7	401283	13	NULL	NULL	0	NULL	NF-kappaB transactivation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of PP2A activity by treatment with okadaic acid or PP2A silencing with small interfering RNA not only enhanced NF-kappaB transactivation but also prevented the increased susceptibility of IEC-TRPC1 cells to apoptosis induced by treatment with tumor necrosis factor-alpha ( TNF-alpha ) / cycloheximide ( CHX ) .
	manualset3
101369	8	401283	13	NULL	NULL	0	NULL	susceptibility	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of PP2A activity by treatment with okadaic acid or PP2A silencing with small interfering RNA not only enhanced NF-kappaB transactivation but also prevented the increased susceptibility of IEC-TRPC1 cells to apoptosis induced by treatment with tumor necrosis factor-alpha ( TNF-alpha ) / cycloheximide ( CHX ) .
	manualset3
101370	9	401283	13	NULL	NULL	0	NULL	IEC-TRPC1 cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of PP2A activity by treatment with okadaic acid or PP2A silencing with small interfering RNA not only enhanced NF-kappaB transactivation but also prevented the increased susceptibility of IEC-TRPC1 cells to apoptosis induced by treatment with tumor necrosis factor-alpha ( TNF-alpha ) / cycloheximide ( CHX ) .
	manualset3
101371	10	401283	13	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of PP2A activity by treatment with okadaic acid or PP2A silencing with small interfering RNA not only enhanced NF-kappaB transactivation but also prevented the increased susceptibility of IEC-TRPC1 cells to apoptosis induced by treatment with tumor necrosis factor-alpha ( TNF-alpha ) / cycloheximide ( CHX ) .
	manualset3
101372	11	401283	13	NULL	NULL	0	NULL	treatment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of PP2A activity by treatment with okadaic acid or PP2A silencing with small interfering RNA not only enhanced NF-kappaB transactivation but also prevented the increased susceptibility of IEC-TRPC1 cells to apoptosis induced by treatment with tumor necrosis factor-alpha ( TNF-alpha ) / cycloheximide ( CHX ) .
	manualset3
101373	12	401283	13	NULL	NULL	0	NULL	tumor necrosis factor-alpha ( TNF-alpha ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of PP2A activity by treatment with okadaic acid or PP2A silencing with small interfering RNA not only enhanced NF-kappaB transactivation but also prevented the increased susceptibility of IEC-TRPC1 cells to apoptosis induced by treatment with tumor necrosis factor-alpha ( TNF-alpha ) / cycloheximide ( CHX ) .
	manualset3
101374	13	401283	13	NULL	NULL	0	NULL	cycloheximide ( CHX ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of PP2A activity by treatment with okadaic acid or PP2A silencing with small interfering RNA not only enhanced NF-kappaB transactivation but also prevented the increased susceptibility of IEC-TRPC1 cells to apoptosis induced by treatment with tumor necrosis factor-alpha ( TNF-alpha ) / cycloheximide ( CHX ) .
	manualset3
101375	1	401284	13	NULL	NULL	0	NULL	Inhibition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of Photosynthesis in Some Algae by Extreme-Red Light .
	manualset3
101376	2	401284	13	NULL	NULL	0	NULL	Photosynthesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of Photosynthesis in Some Algae by Extreme-Red Light .
	manualset3
101377	3	401284	13	NULL	NULL	0	NULL	Algae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of Photosynthesis in Some Algae by Extreme-Red Light .
	manualset3
101378	4	401284	13	NULL	NULL	0	NULL	Extreme-Red Light	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of Photosynthesis in Some Algae by Extreme-Red Light .
	manualset3
101379	1	401285	13	NULL	NULL	0	NULL	Inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of Ras/ERK by a dominant negative Ras or by the MEKI inhibitor , PD98059 , obstructed RET/PTC-mediated apoptosis .
	manualset3
101380	2	401285	13	NULL	NULL	0	NULL	Ras/ERK 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of Ras/ERK by a dominant negative Ras or by the MEKI inhibitor , PD98059 , obstructed RET/PTC-mediated apoptosis .
	manualset3
101381	3	401285	13	NULL	NULL	0	NULL	dominant negative Ras 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of Ras/ERK by a dominant negative Ras or by the MEKI inhibitor , PD98059 , obstructed RET/PTC-mediated apoptosis .
	manualset3
101382	4	401285	13	NULL	NULL	0	NULL	 MEKI inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of Ras/ERK by a dominant negative Ras or by the MEKI inhibitor , PD98059 , obstructed RET/PTC-mediated apoptosis .
	manualset3
101383	5	401285	13	NULL	NULL	0	NULL	PD98059 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of Ras/ERK by a dominant negative Ras or by the MEKI inhibitor , PD98059 , obstructed RET/PTC-mediated apoptosis .
	manualset3
101384	6	401285	13	NULL	NULL	0	NULL	RET/PTC-mediated apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of Ras/ERK by a dominant negative Ras or by the MEKI inhibitor , PD98059 , obstructed RET/PTC-mediated apoptosis .
	manualset3
101385	1	401286	13	NULL	NULL	0	NULL	Association 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	( Association of acquired hemolytic anemia with thrombocytopenic purpura ) .
	manualset3
101386	2	401286	13	NULL	NULL	0	NULL	acquired hemolytic anemia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Association of acquired hemolytic anemia with thrombocytopenic purpura ) .
	manualset3
101387	3	401286	13	NULL	NULL	0	NULL	thrombocytopenic purpura	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Association of acquired hemolytic anemia with thrombocytopenic purpura ) .
	manualset3
101388	1	401287	13	NULL	NULL	0	NULL	Inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of acetylcholine release from motor nerve endings resulting from local anaesthesia by these compounds is suggested as a possible mechanism of their neuromuscular blocking action .
	manualset3
101389	2	401287	13	NULL	NULL	0	NULL	acetylcholine release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of acetylcholine release from motor nerve endings resulting from local anaesthesia by these compounds is suggested as a possible mechanism of their neuromuscular blocking action .
	manualset3
101390	3	401287	13	NULL	NULL	0	NULL	motor nerve endings	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of acetylcholine release from motor nerve endings resulting from local anaesthesia by these compounds is suggested as a possible mechanism of their neuromuscular blocking action .
	manualset3
101391	4	401287	13	NULL	NULL	0	NULL	local anaesthesia	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of acetylcholine release from motor nerve endings resulting from local anaesthesia by these compounds is suggested as a possible mechanism of their neuromuscular blocking action .
	manualset3
101392	5	401287	13	NULL	NULL	0	NULL	compounds 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of acetylcholine release from motor nerve endings resulting from local anaesthesia by these compounds is suggested as a possible mechanism of their neuromuscular blocking action .
	manualset3
101393	6	401287	13	NULL	NULL	0	NULL	possible mechanism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of acetylcholine release from motor nerve endings resulting from local anaesthesia by these compounds is suggested as a possible mechanism of their neuromuscular blocking action .
	manualset3
101394	7	401287	13	NULL	NULL	0	NULL	neuromuscular blocking action	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of acetylcholine release from motor nerve endings resulting from local anaesthesia by these compounds is suggested as a possible mechanism of their neuromuscular blocking action .
	manualset3
101724	1	401288	13	NULL	NULL	0	NULL	Inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of adhesion molecule expression by N-alkylthiopyridine-benzo ( b ) thiophene-2-carboxamides .
	manualset3
101725	2	401288	13	NULL	NULL	0	NULL	adhesion molecule expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of adhesion molecule expression by N-alkylthiopyridine-benzo ( b ) thiophene-2-carboxamides .
	manualset3
101726	3	401288	13	NULL	NULL	0	NULL	N-alkylthiopyridine-benzo ( b ) thiophene-2-carboxamides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of adhesion molecule expression by N-alkylthiopyridine-benzo ( b ) thiophene-2-carboxamides .
	manualset3
101727	1	401289	13	NULL	NULL	0	NULL	Inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of brain prostaglandin synthesis by NCX-2216 ( 22 mg/kg ) persisted for a much longer period of time ( up to 48 h ) than was seen with flurbiprofen ( & lt ; or = 12 h ) .
	manualset3
101728	2	401289	13	NULL	NULL	0	NULL	brain 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of brain prostaglandin synthesis by NCX-2216 ( 22 mg/kg ) persisted for a much longer period of time ( up to 48 h ) than was seen with flurbiprofen ( & lt ; or = 12 h ) .
	manualset3
101729	3	401289	13	NULL	NULL	0	NULL	prostaglandin synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of brain prostaglandin synthesis by NCX-2216 ( 22 mg/kg ) persisted for a much longer period of time ( up to 48 h ) than was seen with flurbiprofen ( & lt ; or = 12 h ) .
	manualset3
101730	4	401289	13	NULL	NULL	0	NULL	NCX-2216	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of brain prostaglandin synthesis by NCX-2216 ( 22 mg/kg ) persisted for a much longer period of time ( up to 48 h ) than was seen with flurbiprofen ( & lt ; or = 12 h ) .
	manualset3
101731	5	401289	13	NULL	NULL	0	NULL	22 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of brain prostaglandin synthesis by NCX-2216 ( 22 mg/kg ) persisted for a much longer period of time ( up to 48 h ) than was seen with flurbiprofen ( & lt ; or = 12 h ) .
	manualset3
101732	6	401289	13	NULL	NULL	0	NULL	period of time 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of brain prostaglandin synthesis by NCX-2216 ( 22 mg/kg ) persisted for a much longer period of time ( up to 48 h ) than was seen with flurbiprofen ( & lt ; or = 12 h ) .
	manualset3
101733	7	401289	13	NULL	NULL	0	NULL	up to 48 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of brain prostaglandin synthesis by NCX-2216 ( 22 mg/kg ) persisted for a much longer period of time ( up to 48 h ) than was seen with flurbiprofen ( & lt ; or = 12 h ) .
	manualset3
101734	8	401289	13	NULL	NULL	0	NULL	flurbiprofen	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of brain prostaglandin synthesis by NCX-2216 ( 22 mg/kg ) persisted for a much longer period of time ( up to 48 h ) than was seen with flurbiprofen ( & lt ; or = 12 h ) .
	manualset3
101735	9	401289	13	NULL	NULL	0	NULL	& lt ; or = 12 h 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of brain prostaglandin synthesis by NCX-2216 ( 22 mg/kg ) persisted for a much longer period of time ( up to 48 h ) than was seen with flurbiprofen ( & lt ; or = 12 h ) .
	manualset3
101736	1	401290	13	NULL	NULL	0	NULL	Inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of cisplatin-induced ATR activity and enhanced sensitivity to cisplatin .
	manualset3
101737	2	401290	13	NULL	NULL	0	NULL	cisplatin-induced ATR activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of cisplatin-induced ATR activity and enhanced sensitivity to cisplatin .
	manualset3
101738	3	401290	13	NULL	NULL	0	NULL	sensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of cisplatin-induced ATR activity and enhanced sensitivity to cisplatin .
	manualset3
101739	4	401290	13	NULL	NULL	0	NULL	cisplatin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of cisplatin-induced ATR activity and enhanced sensitivity to cisplatin .
	manualset3
101740	1	401291	13	NULL	NULL	0	NULL	Inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of cytokine signaling in human retinal endothelial cells through modification of caveolae/lipid rafts by docosahexaenoic acid .
	manualset3
101741	2	401291	13	NULL	NULL	0	NULL	cytokine signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of cytokine signaling in human retinal endothelial cells through modification of caveolae/lipid rafts by docosahexaenoic acid .
	manualset3
101742	3	401291	13	NULL	NULL	0	NULL	human retinal endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of cytokine signaling in human retinal endothelial cells through modification of caveolae/lipid rafts by docosahexaenoic acid .
	manualset3
101743	4	401291	13	NULL	NULL	NULL	NULL	modification 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Inhibition of cytokine signaling in human retinal endothelial cells through modification of caveolae/lipid rafts by docosahexaenoic acid .
	manualset3
101744	5	401291	13	NULL	NULL	0	NULL	caveolae/lipid rafts	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of cytokine signaling in human retinal endothelial cells through modification of caveolae/lipid rafts by docosahexaenoic acid .
	manualset3
101745	6	401291	13	NULL	NULL	0	NULL	 docosahexaenoic acid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of cytokine signaling in human retinal endothelial cells through modification of caveolae/lipid rafts by docosahexaenoic acid .
	manualset3
101746	1	401292	13	NULL	NULL	0	NULL	Inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of drug metabolism by levodopa in combination with a dopa-decarboxylase inhibitor .
	manualset3
101747	2	401292	13	NULL	NULL	0	NULL	drug metabolism 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of drug metabolism by levodopa in combination with a dopa-decarboxylase inhibitor .
	manualset3
101748	3	401292	13	NULL	NULL	0	NULL	levodopa	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of drug metabolism by levodopa in combination with a dopa-decarboxylase inhibitor .
	manualset3
101749	4	401292	13	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of drug metabolism by levodopa in combination with a dopa-decarboxylase inhibitor .
	manualset3
101750	5	401292	13	NULL	NULL	0	NULL	dopa-decarboxylase inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of drug metabolism by levodopa in combination with a dopa-decarboxylase inhibitor .
	manualset3
101751	1	401293	13	NULL	NULL	0	NULL	Inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of estrogen production is therefore a logical treatment strategy .
	manualset3
101752	2	401293	13	NULL	NULL	0	NULL	estrogen production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of estrogen production is therefore a logical treatment strategy .
	manualset3
101753	3	401293	13	NULL	NULL	0	NULL	treatment strategy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of estrogen production is therefore a logical treatment strategy .
	manualset3
101754	1	401294	13	NULL	NULL	0	NULL	Inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of histone H1 kinase expression , retinoblastoma protein phosphorylation , and cell proliferation by the phosphatase inhibitor okadaic acid .
	manualset3
101755	2	401294	13	NULL	NULL	0	NULL	histone H1 kinase expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of histone H1 kinase expression , retinoblastoma protein phosphorylation , and cell proliferation by the phosphatase inhibitor okadaic acid .
	manualset3
101756	3	401294	13	NULL	NULL	0	NULL	retinoblastoma protein phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of histone H1 kinase expression , retinoblastoma protein phosphorylation , and cell proliferation by the phosphatase inhibitor okadaic acid .
	manualset3
101757	4	401294	13	NULL	NULL	0	NULL	cell proliferation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of histone H1 kinase expression , retinoblastoma protein phosphorylation , and cell proliferation by the phosphatase inhibitor okadaic acid .
	manualset3
101758	5	401294	13	NULL	NULL	0	NULL	phosphatase inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of histone H1 kinase expression , retinoblastoma protein phosphorylation , and cell proliferation by the phosphatase inhibitor okadaic acid .
	manualset3
101759	6	401294	13	NULL	NULL	0	NULL	okadaic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of histone H1 kinase expression , retinoblastoma protein phosphorylation , and cell proliferation by the phosphatase inhibitor okadaic acid .
	manualset3
101760	1	401295	13	NULL	NULL	0	NULL	Inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of lysophosphatidic acid receptor-2 expression by RNA interference decreases lysophosphatidic acid-induced urokinase plasminogen activator activation , cell invasion , and migration in ovarian cancer SKOV-3 cells .
	manualset3
101761	2	401295	13	NULL	NULL	0	NULL	lysophosphatidic acid receptor-2 expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of lysophosphatidic acid receptor-2 expression by RNA interference decreases lysophosphatidic acid-induced urokinase plasminogen activator activation , cell invasion , and migration in ovarian cancer SKOV-3 cells .
	manualset3
101762	3	401295	13	NULL	NULL	0	NULL	RNA interference 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of lysophosphatidic acid receptor-2 expression by RNA interference decreases lysophosphatidic acid-induced urokinase plasminogen activator activation , cell invasion , and migration in ovarian cancer SKOV-3 cells .
	manualset3
101763	4	401295	13	NULL	NULL	0	NULL	lysophosphatidic acid-induced urokinase plasminogen activator activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of lysophosphatidic acid receptor-2 expression by RNA interference decreases lysophosphatidic acid-induced urokinase plasminogen activator activation , cell invasion , and migration in ovarian cancer SKOV-3 cells .
	manualset3
101764	5	401295	13	NULL	NULL	0	NULL	cell invasion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of lysophosphatidic acid receptor-2 expression by RNA interference decreases lysophosphatidic acid-induced urokinase plasminogen activator activation , cell invasion , and migration in ovarian cancer SKOV-3 cells .
	manualset3
101765	6	401295	13	NULL	NULL	0	NULL	migration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of lysophosphatidic acid receptor-2 expression by RNA interference decreases lysophosphatidic acid-induced urokinase plasminogen activator activation , cell invasion , and migration in ovarian cancer SKOV-3 cells .
	manualset3
101766	7	401295	13	NULL	NULL	0	NULL	ovarian cancer SKOV-3 cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of lysophosphatidic acid receptor-2 expression by RNA interference decreases lysophosphatidic acid-induced urokinase plasminogen activator activation , cell invasion , and migration in ovarian cancer SKOV-3 cells .
	manualset3
101767	1	401296	13	NULL	NULL	0	NULL	Inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of soluble epoxide hydrolase ( SEH ) , the enzyme responsible for degradation of vasoactive epoxides , protects against cerebral ischemia in rats .
	manualset3
101768	2	401296	13	NULL	NULL	0	NULL	soluble epoxide hydrolase ( SEH ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of soluble epoxide hydrolase ( SEH ) , the enzyme responsible for degradation of vasoactive epoxides , protects against cerebral ischemia in rats .
	manualset3
101769	3	401296	13	NULL	NULL	0	NULL	 enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of soluble epoxide hydrolase ( SEH ) , the enzyme responsible for degradation of vasoactive epoxides , protects against cerebral ischemia in rats .
	manualset3
101770	4	401296	13	NULL	NULL	0	NULL	degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of soluble epoxide hydrolase ( SEH ) , the enzyme responsible for degradation of vasoactive epoxides , protects against cerebral ischemia in rats .
	manualset3
101771	5	401296	13	NULL	NULL	0	NULL	vasoactive epoxides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of soluble epoxide hydrolase ( SEH ) , the enzyme responsible for degradation of vasoactive epoxides , protects against cerebral ischemia in rats .
	manualset3
101772	6	401296	13	NULL	NULL	0	NULL	cerebral ischemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of soluble epoxide hydrolase ( SEH ) , the enzyme responsible for degradation of vasoactive epoxides , protects against cerebral ischemia in rats .
	manualset3
101773	7	401296	13	NULL	NULL	0	NULL	 rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of soluble epoxide hydrolase ( SEH ) , the enzyme responsible for degradation of vasoactive epoxides , protects against cerebral ischemia in rats .
	manualset3
101774	1	401297	13	NULL	NULL	0	NULL	Inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of stimulated oxytocin release was only produced in group B. These findings suggest that the inhibitory effect of melatonin depends on the time of day and are consistent with the suggestion that melatonin secretion during the dark period may acutely downregulate binding sites in the brain .
	manualset3
101775	2	401297	13	NULL	NULL	0	NULL	 oxytocin release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of stimulated oxytocin release was only produced in group B. These findings suggest that the inhibitory effect of melatonin depends on the time of day and are consistent with the suggestion that melatonin secretion during the dark period may acutely downregulate binding sites in the brain .
	manualset3
101776	3	401297	13	NULL	NULL	0	NULL	group B	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of stimulated oxytocin release was only produced in group B. These findings suggest that the inhibitory effect of melatonin depends on the time of day and are consistent with the suggestion that melatonin secretion during the dark period may acutely downregulate binding sites in the brain .
	manualset3
101777	4	401297	13	NULL	NULL	0	NULL	findings	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of stimulated oxytocin release was only produced in group B. These findings suggest that the inhibitory effect of melatonin depends on the time of day and are consistent with the suggestion that melatonin secretion during the dark period may acutely downregulate binding sites in the brain .
	manualset3
101778	5	401297	13	NULL	NULL	0	NULL	inhibitory effect 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of stimulated oxytocin release was only produced in group B. These findings suggest that the inhibitory effect of melatonin depends on the time of day and are consistent with the suggestion that melatonin secretion during the dark period may acutely downregulate binding sites in the brain .
	manualset3
101779	6	401297	13	NULL	NULL	0	NULL	melatonin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of stimulated oxytocin release was only produced in group B. These findings suggest that the inhibitory effect of melatonin depends on the time of day and are consistent with the suggestion that melatonin secretion during the dark period may acutely downregulate binding sites in the brain .
	manualset3
101780	7	401297	13	NULL	NULL	0	NULL	 time of day	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of stimulated oxytocin release was only produced in group B. These findings suggest that the inhibitory effect of melatonin depends on the time of day and are consistent with the suggestion that melatonin secretion during the dark period may acutely downregulate binding sites in the brain .
	manualset3
101781	8	401297	13	NULL	NULL	0	NULL	suggestion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of stimulated oxytocin release was only produced in group B. These findings suggest that the inhibitory effect of melatonin depends on the time of day and are consistent with the suggestion that melatonin secretion during the dark period may acutely downregulate binding sites in the brain .
	manualset3
101782	9	401297	13	NULL	NULL	0	NULL	melatonin secretion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of stimulated oxytocin release was only produced in group B. These findings suggest that the inhibitory effect of melatonin depends on the time of day and are consistent with the suggestion that melatonin secretion during the dark period may acutely downregulate binding sites in the brain .
	manualset3
101783	10	401297	13	NULL	NULL	0	NULL	dark period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of stimulated oxytocin release was only produced in group B. These findings suggest that the inhibitory effect of melatonin depends on the time of day and are consistent with the suggestion that melatonin secretion during the dark period may acutely downregulate binding sites in the brain .
	manualset3
101784	11	401297	13	NULL	NULL	0	NULL	binding sites	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of stimulated oxytocin release was only produced in group B. These findings suggest that the inhibitory effect of melatonin depends on the time of day and are consistent with the suggestion that melatonin secretion during the dark period may acutely downregulate binding sites in the brain .
	manualset3
101785	12	401297	13	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of stimulated oxytocin release was only produced in group B. These findings suggest that the inhibitory effect of melatonin depends on the time of day and are consistent with the suggestion that melatonin secretion during the dark period may acutely downregulate binding sites in the brain .
	manualset3
101786	1	401298	13	NULL	NULL	0	NULL	Inhibition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of sympathetic nerve activity by acute administration of the tricyclic antidepressant desipramine .
	manualset3
101787	2	401298	13	NULL	NULL	0	NULL	sympathetic nerve activity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of sympathetic nerve activity by acute administration of the tricyclic antidepressant desipramine .
	manualset3
101788	3	401298	13	NULL	NULL	0	NULL	acute administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of sympathetic nerve activity by acute administration of the tricyclic antidepressant desipramine .
	manualset3
101789	4	401298	13	NULL	NULL	0	NULL	tricyclic antidepressant desipramine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of sympathetic nerve activity by acute administration of the tricyclic antidepressant desipramine .
	manualset3
101790	1	401299	13	NULL	NULL	NULL	NULL	Inhibition	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Inhibition of synthesis of sulfated mucopolysaccharides by estradiol .
	manualset3
101791	2	401299	13	NULL	NULL	NULL	NULL	synthesis of sulfated mucopolysaccharides	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Inhibition of synthesis of sulfated mucopolysaccharides by estradiol .
	manualset3
101792	3	401299	13	NULL	NULL	0	NULL	estradiol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of synthesis of sulfated mucopolysaccharides by estradiol .
	manualset3
101793	1	401300	13	NULL	NULL	0	NULL	Inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of the primary in vitro antibody response by interferon preparations .
	manualset3
101794	2	401300	13	NULL	NULL	0	NULL	 primary in vitro antibody response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of the primary in vitro antibody response by interferon preparations .
	manualset3
101795	3	401300	13	NULL	NULL	0	NULL	interferon preparations	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of the primary in vitro antibody response by interferon preparations .
	manualset3
101796	1	401301	13	NULL	NULL	0	NULL	Inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of virus replication in our system is dependent upon the specificity of the Ab for the viral protein .
	manualset3
101797	2	401301	13	NULL	NULL	0	NULL	virus replication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of virus replication in our system is dependent upon the specificity of the Ab for the viral protein .
	manualset3
101798	3	401301	13	NULL	NULL	0	NULL	our system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of virus replication in our system is dependent upon the specificity of the Ab for the viral protein .
	manualset3
101799	4	401301	13	NULL	NULL	0	NULL	specificity of the Ab	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of virus replication in our system is dependent upon the specificity of the Ab for the viral protein .
	manualset3
101800	5	401301	13	NULL	NULL	0	NULL	 viral protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of virus replication in our system is dependent upon the specificity of the Ab for the viral protein .
	manualset3
101801	1	401302	13	NULL	NULL	0	NULL	Inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of white spot syndrome virus replication in Penaeus monodon by combined silencing of viral rr2 and shrimp PmRab7 .
	manualset3
101802	2	401302	13	NULL	NULL	0	NULL	white spot syndrome virus replication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of white spot syndrome virus replication in Penaeus monodon by combined silencing of viral rr2 and shrimp PmRab7 .
	manualset3
101803	3	401302	13	NULL	NULL	0	NULL	 Penaeus monodon	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of white spot syndrome virus replication in Penaeus monodon by combined silencing of viral rr2 and shrimp PmRab7 .
	manualset3
101804	4	401302	13	NULL	NULL	NULL	NULL	viral rr2	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Inhibition of white spot syndrome virus replication in Penaeus monodon by combined silencing of viral rr2 and shrimp PmRab7 .
	manualset3
101805	5	401302	13	NULL	NULL	NULL	NULL	 shrimp PmRab7	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Inhibition of white spot syndrome virus replication in Penaeus monodon by combined silencing of viral rr2 and shrimp PmRab7 .
	manualset3
101806	1	401303	13	NULL	NULL	0	NULL	Inhibition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition was also observed with quinidine ( 1 mM ) and lignocaine ( 10 - minus 2 M ) .
	manualset3
101807	2	401303	13	NULL	NULL	0	NULL	quinidine ( 1 mM )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition was also observed with quinidine ( 1 mM ) and lignocaine ( 10 - minus 2 M ) .
	manualset3
101808	3	401303	13	NULL	NULL	0	NULL	 lignocaine ( 10 - minus 2 M ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition was also observed with quinidine ( 1 mM ) and lignocaine ( 10 - minus 2 M ) .
	manualset3
101809	1	401304	13	NULL	NULL	NULL	NULL	Inhibitors of EMP enzymes	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Inhibitors of EMP enzymes restricted vegetative growth more than that associated with conidiation whilst arsenate augmented the limited capacity of lower levels of Ca2 + to promote conidiation .
	manualset3
101810	2	401304	13	NULL	NULL	0	NULL	vegetative growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibitors of EMP enzymes restricted vegetative growth more than that associated with conidiation whilst arsenate augmented the limited capacity of lower levels of Ca2 + to promote conidiation .
	manualset3
101811	3	401304	13	NULL	NULL	0	NULL	conidiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibitors of EMP enzymes restricted vegetative growth more than that associated with conidiation whilst arsenate augmented the limited capacity of lower levels of Ca2 + to promote conidiation .
	manualset3
101812	4	401304	13	NULL	NULL	NULL	NULL	arsenate	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Inhibitors of EMP enzymes restricted vegetative growth more than that associated with conidiation whilst arsenate augmented the limited capacity of lower levels of Ca2 + to promote conidiation .
	manualset3
101813	5	401304	13	NULL	NULL	0	NULL	capacity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibitors of EMP enzymes restricted vegetative growth more than that associated with conidiation whilst arsenate augmented the limited capacity of lower levels of Ca2 + to promote conidiation .
	manualset3
101814	6	401304	13	NULL	NULL	0	NULL	lower levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibitors of EMP enzymes restricted vegetative growth more than that associated with conidiation whilst arsenate augmented the limited capacity of lower levels of Ca2 + to promote conidiation .
	manualset3
101815	7	401304	13	NULL	NULL	0	NULL	Ca2 + 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibitors of EMP enzymes restricted vegetative growth more than that associated with conidiation whilst arsenate augmented the limited capacity of lower levels of Ca2 + to promote conidiation .
	manualset3
101816	8	401304	13	NULL	NULL	0	NULL	conidiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibitors of EMP enzymes restricted vegetative growth more than that associated with conidiation whilst arsenate augmented the limited capacity of lower levels of Ca2 + to promote conidiation .
	manualset3
101817	1	401305	13	NULL	NULL	0	NULL	Inhibitory activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibitory activity of plumbagin produced by Drosera intermedia on food spoilage fungi .
	manualset3
101818	2	401305	13	NULL	NULL	0	NULL	plumbagin 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibitory activity of plumbagin produced by Drosera intermedia on food spoilage fungi .
	manualset3
101819	3	401305	13	NULL	NULL	0	NULL	Drosera intermedia	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibitory activity of plumbagin produced by Drosera intermedia on food spoilage fungi .
	manualset3
101820	4	401305	13	NULL	NULL	0	NULL	food spoilage fungi	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibitory activity of plumbagin produced by Drosera intermedia on food spoilage fungi .
	manualset3
101821	1	401306	13	NULL	NULL	0	NULL	3 , 4-DHPEA 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	3 , 4-DHPEA showed a potent inhibitory activity on DNA synthesis , as evidenced by a 92 % reduction of ( 3H ) - thymidine incorporation at 100 micromol/L , and an induced apoptosis , as evidenced by the release of cytosolic nucleosomes and flow cytometry .
	manualset3
101822	2	401306	13	NULL	NULL	0	NULL	inhibitory activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	3 , 4-DHPEA showed a potent inhibitory activity on DNA synthesis , as evidenced by a 92 % reduction of ( 3H ) - thymidine incorporation at 100 micromol/L , and an induced apoptosis , as evidenced by the release of cytosolic nucleosomes and flow cytometry .
	manualset3
101823	3	401306	13	NULL	NULL	0	NULL	DNA synthesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	3 , 4-DHPEA showed a potent inhibitory activity on DNA synthesis , as evidenced by a 92 % reduction of ( 3H ) - thymidine incorporation at 100 micromol/L , and an induced apoptosis , as evidenced by the release of cytosolic nucleosomes and flow cytometry .
	manualset3
101824	4	401306	13	NULL	NULL	0	NULL	92 % reduction	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	3 , 4-DHPEA showed a potent inhibitory activity on DNA synthesis , as evidenced by a 92 % reduction of ( 3H ) - thymidine incorporation at 100 micromol/L , and an induced apoptosis , as evidenced by the release of cytosolic nucleosomes and flow cytometry .
	manualset3
101825	5	401306	13	NULL	NULL	0	NULL	( 3H ) - thymidine incorporation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	3 , 4-DHPEA showed a potent inhibitory activity on DNA synthesis , as evidenced by a 92 % reduction of ( 3H ) - thymidine incorporation at 100 micromol/L , and an induced apoptosis , as evidenced by the release of cytosolic nucleosomes and flow cytometry .
	manualset3
101826	6	401306	13	NULL	NULL	0	NULL	100 micromol/L 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	3 , 4-DHPEA showed a potent inhibitory activity on DNA synthesis , as evidenced by a 92 % reduction of ( 3H ) - thymidine incorporation at 100 micromol/L , and an induced apoptosis , as evidenced by the release of cytosolic nucleosomes and flow cytometry .
	manualset3
101827	7	401306	13	NULL	NULL	0	NULL	apoptosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	3 , 4-DHPEA showed a potent inhibitory activity on DNA synthesis , as evidenced by a 92 % reduction of ( 3H ) - thymidine incorporation at 100 micromol/L , and an induced apoptosis , as evidenced by the release of cytosolic nucleosomes and flow cytometry .
	manualset3
101828	8	401306	13	NULL	NULL	0	NULL	release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	3 , 4-DHPEA showed a potent inhibitory activity on DNA synthesis , as evidenced by a 92 % reduction of ( 3H ) - thymidine incorporation at 100 micromol/L , and an induced apoptosis , as evidenced by the release of cytosolic nucleosomes and flow cytometry .
	manualset3
101829	9	401306	13	NULL	NULL	0	NULL	cytosolic nucleosomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	3 , 4-DHPEA showed a potent inhibitory activity on DNA synthesis , as evidenced by a 92 % reduction of ( 3H ) - thymidine incorporation at 100 micromol/L , and an induced apoptosis , as evidenced by the release of cytosolic nucleosomes and flow cytometry .
	manualset3
101830	10	401306	13	NULL	NULL	0	NULL	flow cytometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	3 , 4-DHPEA showed a potent inhibitory activity on DNA synthesis , as evidenced by a 92 % reduction of ( 3H ) - thymidine incorporation at 100 micromol/L , and an induced apoptosis , as evidenced by the release of cytosolic nucleosomes and flow cytometry .
	manualset3
101831	1	401307	13	NULL	NULL	0	NULL	Inhibitory effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibitory effects of the quinolone antibiotics ofloxacin , lomefloxacin , pipemidic acid , ciprofloxacin , and enoxacin on caffeine metabolism were examined in vitro with human liver microsomes of four donors .
	manualset3
101832	2	401307	13	NULL	NULL	0	NULL	quinolone antibiotics 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibitory effects of the quinolone antibiotics ofloxacin , lomefloxacin , pipemidic acid , ciprofloxacin , and enoxacin on caffeine metabolism were examined in vitro with human liver microsomes of four donors .
	manualset3
101833	3	401307	13	NULL	NULL	0	NULL	ofloxacin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibitory effects of the quinolone antibiotics ofloxacin , lomefloxacin , pipemidic acid , ciprofloxacin , and enoxacin on caffeine metabolism were examined in vitro with human liver microsomes of four donors .
	manualset3
101834	4	401307	13	NULL	NULL	0	NULL	lomefloxacin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibitory effects of the quinolone antibiotics ofloxacin , lomefloxacin , pipemidic acid , ciprofloxacin , and enoxacin on caffeine metabolism were examined in vitro with human liver microsomes of four donors .
	manualset3
101835	5	401307	13	NULL	NULL	0	NULL	pipemidic acid	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibitory effects of the quinolone antibiotics ofloxacin , lomefloxacin , pipemidic acid , ciprofloxacin , and enoxacin on caffeine metabolism were examined in vitro with human liver microsomes of four donors .
	manualset3
101836	6	401307	13	NULL	NULL	0	NULL	ciprofloxacin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibitory effects of the quinolone antibiotics ofloxacin , lomefloxacin , pipemidic acid , ciprofloxacin , and enoxacin on caffeine metabolism were examined in vitro with human liver microsomes of four donors .
	manualset3
101837	7	401307	13	NULL	NULL	0	NULL	enoxacin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibitory effects of the quinolone antibiotics ofloxacin , lomefloxacin , pipemidic acid , ciprofloxacin , and enoxacin on caffeine metabolism were examined in vitro with human liver microsomes of four donors .
	manualset3
101838	8	401307	13	NULL	NULL	0	NULL	caffeine metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibitory effects of the quinolone antibiotics ofloxacin , lomefloxacin , pipemidic acid , ciprofloxacin , and enoxacin on caffeine metabolism were examined in vitro with human liver microsomes of four donors .
	manualset3
101839	9	401307	13	NULL	NULL	0	NULL	human liver microsomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibitory effects of the quinolone antibiotics ofloxacin , lomefloxacin , pipemidic acid , ciprofloxacin , and enoxacin on caffeine metabolism were examined in vitro with human liver microsomes of four donors .
	manualset3
101840	10	401307	13	NULL	NULL	0	NULL	four donors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibitory effects of the quinolone antibiotics ofloxacin , lomefloxacin , pipemidic acid , ciprofloxacin , and enoxacin on caffeine metabolism were examined in vitro with human liver microsomes of four donors .
	manualset3
101841	1	401308	13	NULL	NULL	0	NULL	Initial findings 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial findings demonstrate the high levels of stress experienced by staff , related to emotional labor and to conflicts around the erosion of care standards .
	manualset3
101842	2	401308	13	NULL	NULL	0	NULL	high levels of stress 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial findings demonstrate the high levels of stress experienced by staff , related to emotional labor and to conflicts around the erosion of care standards .
	manualset3
101843	3	401308	13	NULL	NULL	0	NULL	staff 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial findings demonstrate the high levels of stress experienced by staff , related to emotional labor and to conflicts around the erosion of care standards .
	manualset3
101844	4	401308	13	NULL	NULL	0	NULL	emotional labor 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial findings demonstrate the high levels of stress experienced by staff , related to emotional labor and to conflicts around the erosion of care standards .
	manualset3
101845	5	401308	13	NULL	NULL	0	NULL	conflicts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial findings demonstrate the high levels of stress experienced by staff , related to emotional labor and to conflicts around the erosion of care standards .
	manualset3
101846	6	401308	13	NULL	NULL	0	NULL	erosion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial findings demonstrate the high levels of stress experienced by staff , related to emotional labor and to conflicts around the erosion of care standards .
	manualset3
101847	7	401308	13	NULL	NULL	0	NULL	care standards	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial findings demonstrate the high levels of stress experienced by staff , related to emotional labor and to conflicts around the erosion of care standards .
	manualset3
101848	1	401309	13	NULL	NULL	NULL	NULL	Initial fixation 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Initial fixation in glutaraldehyde followed by postfixation in osmium-antimonate solutions provided better preservation of structure but less precipitation than direct fixation in osmium-antimonate .
	manualset3
101849	2	401309	13	NULL	NULL	0	NULL	glutaraldehyde	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial fixation in glutaraldehyde followed by postfixation in osmium-antimonate solutions provided better preservation of structure but less precipitation than direct fixation in osmium-antimonate .
	manualset3
101850	3	401309	13	NULL	NULL	0	NULL	postfixation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial fixation in glutaraldehyde followed by postfixation in osmium-antimonate solutions provided better preservation of structure but less precipitation than direct fixation in osmium-antimonate .
	manualset3
101851	4	401309	13	NULL	NULL	0	NULL	osmium-antimonate solutions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial fixation in glutaraldehyde followed by postfixation in osmium-antimonate solutions provided better preservation of structure but less precipitation than direct fixation in osmium-antimonate .
	manualset3
101852	5	401309	13	NULL	NULL	0	NULL	preservation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial fixation in glutaraldehyde followed by postfixation in osmium-antimonate solutions provided better preservation of structure but less precipitation than direct fixation in osmium-antimonate .
	manualset3
101853	6	401309	13	NULL	NULL	0	NULL	structure 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial fixation in glutaraldehyde followed by postfixation in osmium-antimonate solutions provided better preservation of structure but less precipitation than direct fixation in osmium-antimonate .
	manualset3
101854	7	401309	13	NULL	NULL	0	NULL	precipitation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial fixation in glutaraldehyde followed by postfixation in osmium-antimonate solutions provided better preservation of structure but less precipitation than direct fixation in osmium-antimonate .
	manualset3
101855	8	401309	13	NULL	NULL	0	NULL	direct fixation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial fixation in glutaraldehyde followed by postfixation in osmium-antimonate solutions provided better preservation of structure but less precipitation than direct fixation in osmium-antimonate .
	manualset3
101856	9	401309	13	NULL	NULL	0	NULL	osmium-antimonate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial fixation in glutaraldehyde followed by postfixation in osmium-antimonate solutions provided better preservation of structure but less precipitation than direct fixation in osmium-antimonate .
	manualset3
101857	1	401310	13	NULL	NULL	0	NULL	Initial impressions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial impressions of the program are presented .
	manualset3
101858	2	401310	13	NULL	NULL	0	NULL	program 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial impressions of the program are presented .
	manualset3
101859	1	401311	13	NULL	NULL	0	NULL	Initial management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial management of minor and moderate , uncomplicated burn injury focuses on wound management and patient comfort .
	manualset3
101860	2	401311	13	NULL	NULL	0	NULL	minor burn injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial management of minor and moderate , uncomplicated burn injury focuses on wound management and patient comfort .
	manualset3
101861	3	401311	13	NULL	NULL	0	NULL	moderate burn injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial management of minor and moderate , uncomplicated burn injury focuses on wound management and patient comfort .
	manualset3
101862	4	401311	13	NULL	NULL	0	NULL	uncomplicated burn injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial management of minor and moderate , uncomplicated burn injury focuses on wound management and patient comfort .
	manualset3
101863	5	401311	13	NULL	NULL	0	NULL	wound management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial management of minor and moderate , uncomplicated burn injury focuses on wound management and patient comfort .
	manualset3
101864	6	401311	13	NULL	NULL	0	NULL	 patient comfort	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial management of minor and moderate , uncomplicated burn injury focuses on wound management and patient comfort .
	manualset3
101865	1	401312	13	NULL	NULL	0	NULL	Initial velocity studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial velocity studies revealed that FB ( 1 ) is a total uncompetitive inhibitor of this enzyme with an inhibition constant value of 17.5 + / -1 microM .
	manualset3
101866	2	401312	13	NULL	NULL	0	NULL	FB ( 1 ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial velocity studies revealed that FB ( 1 ) is a total uncompetitive inhibitor of this enzyme with an inhibition constant value of 17.5 + / -1 microM .
	manualset3
101867	3	401312	13	NULL	NULL	0	NULL	total uncompetitive inhibitor 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial velocity studies revealed that FB ( 1 ) is a total uncompetitive inhibitor of this enzyme with an inhibition constant value of 17.5 + / -1 microM .
	manualset3
101868	4	401312	13	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial velocity studies revealed that FB ( 1 ) is a total uncompetitive inhibitor of this enzyme with an inhibition constant value of 17.5 + / -1 microM .
	manualset3
101869	5	401312	13	NULL	NULL	0	NULL	inhibition constant value	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial velocity studies revealed that FB ( 1 ) is a total uncompetitive inhibitor of this enzyme with an inhibition constant value of 17.5 + / -1 microM .
	manualset3
101870	6	401312	13	NULL	NULL	0	NULL	17.5 + / -1 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial velocity studies revealed that FB ( 1 ) is a total uncompetitive inhibitor of this enzyme with an inhibition constant value of 17.5 + / -1 microM .
	manualset3
101871	1	401313	13	NULL	NULL	0	NULL	16 mg 6-OHDA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Initially , 16 mg 6-OHDA ( 6-OHDA group ) or vehicle ( artificial cerebrospinal fluid - aCSF ; Sham group ) was infused into the right MFB of adult male Wistar rats .
	manualset3
101872	2	401313	13	NULL	NULL	0	NULL	6-OHDA group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Initially , 16 mg 6-OHDA ( 6-OHDA group ) or vehicle ( artificial cerebrospinal fluid - aCSF ; Sham group ) was infused into the right MFB of adult male Wistar rats .
	manualset3
101873	3	401313	13	NULL	NULL	0	NULL	vehicle	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Initially , 16 mg 6-OHDA ( 6-OHDA group ) or vehicle ( artificial cerebrospinal fluid - aCSF ; Sham group ) was infused into the right MFB of adult male Wistar rats .
	manualset3
101874	4	401313	13	NULL	NULL	0	NULL	artificial cerebrospinal fluid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Initially , 16 mg 6-OHDA ( 6-OHDA group ) or vehicle ( artificial cerebrospinal fluid - aCSF ; Sham group ) was infused into the right MFB of adult male Wistar rats .
	manualset3
101875	5	401313	13	NULL	NULL	0	NULL	aCSF	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Initially , 16 mg 6-OHDA ( 6-OHDA group ) or vehicle ( artificial cerebrospinal fluid - aCSF ; Sham group ) was infused into the right MFB of adult male Wistar rats .
	manualset3
101876	6	401313	13	NULL	NULL	0	NULL	Sham group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Initially , 16 mg 6-OHDA ( 6-OHDA group ) or vehicle ( artificial cerebrospinal fluid - aCSF ; Sham group ) was infused into the right MFB of adult male Wistar rats .
	manualset3
101877	7	401313	13	NULL	NULL	0	NULL	right MFB	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Initially , 16 mg 6-OHDA ( 6-OHDA group ) or vehicle ( artificial cerebrospinal fluid - aCSF ; Sham group ) was infused into the right MFB of adult male Wistar rats .
	manualset3
101878	8	401313	13	NULL	NULL	0	NULL	adult male Wistar rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Initially , 16 mg 6-OHDA ( 6-OHDA group ) or vehicle ( artificial cerebrospinal fluid - aCSF ; Sham group ) was infused into the right MFB of adult male Wistar rats .
	manualset3
101879	1	401314	13	NULL	NULL	0	NULL	increase ( fivefold ) 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Initially , there was a significant increase ( fivefold ) in the peripheral white blood count ( WBC ) , including a 10-fold rise in the absolute neutrophil count .
	manualset3
101880	2	401314	13	NULL	NULL	0	NULL	peripheral white blood count ( WBC )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Initially , there was a significant increase ( fivefold ) in the peripheral white blood count ( WBC ) , including a 10-fold rise in the absolute neutrophil count .
	manualset3
101881	3	401314	13	NULL	NULL	0	NULL	10-fold rise	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Initially , there was a significant increase ( fivefold ) in the peripheral white blood count ( WBC ) , including a 10-fold rise in the absolute neutrophil count .
	manualset3
101882	4	401314	13	NULL	NULL	0	NULL	neutrophil count 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Initially , there was a significant increase ( fivefold ) in the peripheral white blood count ( WBC ) , including a 10-fold rise in the absolute neutrophil count .
	manualset3
101883	1	401315	13	NULL	NULL	0	NULL	3 , 4 chlorcresol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	3 , 4 chlorcresol , instead , is able to retard the begin and reduce the amount of decomposition in concentrations , which were found as maximal concentrations for phenolic substances in the sewage samples .
	manualset3
101884	2	401315	13	NULL	NULL	0	NULL	amount of decomposition	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	3 , 4 chlorcresol , instead , is able to retard the begin and reduce the amount of decomposition in concentrations , which were found as maximal concentrations for phenolic substances in the sewage samples .
	manualset3
101885	3	401315	13	NULL	NULL	0	NULL	concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	3 , 4 chlorcresol , instead , is able to retard the begin and reduce the amount of decomposition in concentrations , which were found as maximal concentrations for phenolic substances in the sewage samples .
	manualset3
101886	4	401315	13	NULL	NULL	0	NULL	maximal concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	3 , 4 chlorcresol , instead , is able to retard the begin and reduce the amount of decomposition in concentrations , which were found as maximal concentrations for phenolic substances in the sewage samples .
	manualset3
101887	5	401315	13	NULL	NULL	0	NULL	phenolic substances 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	3 , 4 chlorcresol , instead , is able to retard the begin and reduce the amount of decomposition in concentrations , which were found as maximal concentrations for phenolic substances in the sewage samples .
	manualset3
101888	6	401315	13	NULL	NULL	0	NULL	sewage samples	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	3 , 4 chlorcresol , instead , is able to retard the begin and reduce the amount of decomposition in concentrations , which were found as maximal concentrations for phenolic substances in the sewage samples .
	manualset3
101889	1	401316	13	NULL	NULL	0	NULL	forty-six	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Initially , there were forty-six open fractures and four closed fractures with a compartment syndrome .
	manualset3
101890	2	401316	13	NULL	NULL	0	NULL	open fractures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Initially , there were forty-six open fractures and four closed fractures with a compartment syndrome .
	manualset3
101891	3	401316	13	NULL	NULL	0	NULL	four	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Initially , there were forty-six open fractures and four closed fractures with a compartment syndrome .
	manualset3
101892	4	401316	13	NULL	NULL	0	NULL	closed fractures 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Initially , there were forty-six open fractures and four closed fractures with a compartment syndrome .
	manualset3
101893	5	401316	13	NULL	NULL	0	NULL	compartment syndrome 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Initially , there were forty-six open fractures and four closed fractures with a compartment syndrome .
	manualset3
101894	1	401317	13	NULL	NULL	0	NULL	human autoimmune serum	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Initially the human autoimmune serum was used to select a cDNA of 317 amino acids from a hamster expression library .
	manualset3
101895	2	401317	13	NULL	NULL	0	NULL	cDNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Initially the human autoimmune serum was used to select a cDNA of 317 amino acids from a hamster expression library .
	manualset3
101896	3	401317	13	NULL	NULL	0	NULL	317 amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Initially the human autoimmune serum was used to select a cDNA of 317 amino acids from a hamster expression library .
	manualset3
101897	4	401317	13	NULL	NULL	0	NULL	hamster expression library	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Initially the human autoimmune serum was used to select a cDNA of 317 amino acids from a hamster expression library .
	manualset3
101898	1	401318	13	NULL	NULL	0	NULL	Initiation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Initiation of vascular MCI pathology was not associated with loss of neurons , but was correlated with microglial activation and white matter changes .
	manualset3
101899	2	401318	13	NULL	NULL	0	NULL	vascular MCI pathology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Initiation of vascular MCI pathology was not associated with loss of neurons , but was correlated with microglial activation and white matter changes .
	manualset3
101900	3	401318	13	NULL	NULL	0	NULL	loss of neurons	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Initiation of vascular MCI pathology was not associated with loss of neurons , but was correlated with microglial activation and white matter changes .
	manualset3
101901	4	401318	13	NULL	NULL	0	NULL	microglial activation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Initiation of vascular MCI pathology was not associated with loss of neurons , but was correlated with microglial activation and white matter changes .
	manualset3
101902	5	401318	13	NULL	NULL	0	NULL	white matter changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Initiation of vascular MCI pathology was not associated with loss of neurons , but was correlated with microglial activation and white matter changes .
	manualset3
101903	1	401319	13	NULL	NULL	0	NULL	Initiatives	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Initiatives such as these are producing positive changes within healthcare organizations , but two serious barriers all but preclude improvement at the system level : a compensation process that punishes innovation and the emergence of integrated care systems that lack a common vision .
	manualset3
101904	2	401319	13	NULL	NULL	0	NULL	positive changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Initiatives such as these are producing positive changes within healthcare organizations , but two serious barriers all but preclude improvement at the system level : a compensation process that punishes innovation and the emergence of integrated care systems that lack a common vision .
	manualset3
101905	3	401319	13	NULL	NULL	0	NULL	healthcare organizations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Initiatives such as these are producing positive changes within healthcare organizations , but two serious barriers all but preclude improvement at the system level : a compensation process that punishes innovation and the emergence of integrated care systems that lack a common vision .
	manualset3
101906	4	401319	13	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Initiatives such as these are producing positive changes within healthcare organizations , but two serious barriers all but preclude improvement at the system level : a compensation process that punishes innovation and the emergence of integrated care systems that lack a common vision .
	manualset3
101907	5	401319	13	NULL	NULL	0	NULL	serious barriers	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Initiatives such as these are producing positive changes within healthcare organizations , but two serious barriers all but preclude improvement at the system level : a compensation process that punishes innovation and the emergence of integrated care systems that lack a common vision .
	manualset3
101908	6	401319	13	NULL	NULL	0	NULL	improvement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Initiatives such as these are producing positive changes within healthcare organizations , but two serious barriers all but preclude improvement at the system level : a compensation process that punishes innovation and the emergence of integrated care systems that lack a common vision .
	manualset3
101909	7	401319	13	NULL	NULL	0	NULL	system level 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Initiatives such as these are producing positive changes within healthcare organizations , but two serious barriers all but preclude improvement at the system level : a compensation process that punishes innovation and the emergence of integrated care systems that lack a common vision .
	manualset3
101910	8	401319	13	NULL	NULL	0	NULL	compensation process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Initiatives such as these are producing positive changes within healthcare organizations , but two serious barriers all but preclude improvement at the system level : a compensation process that punishes innovation and the emergence of integrated care systems that lack a common vision .
	manualset3
101911	9	401319	13	NULL	NULL	0	NULL	 innovation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Initiatives such as these are producing positive changes within healthcare organizations , but two serious barriers all but preclude improvement at the system level : a compensation process that punishes innovation and the emergence of integrated care systems that lack a common vision .
	manualset3
101912	10	401319	13	NULL	NULL	0	NULL	emergence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Initiatives such as these are producing positive changes within healthcare organizations , but two serious barriers all but preclude improvement at the system level : a compensation process that punishes innovation and the emergence of integrated care systems that lack a common vision .
	manualset3
101913	11	401319	13	NULL	NULL	0	NULL	care systems 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Initiatives such as these are producing positive changes within healthcare organizations , but two serious barriers all but preclude improvement at the system level : a compensation process that punishes innovation and the emergence of integrated care systems that lack a common vision .
	manualset3
101914	12	401319	13	NULL	NULL	0	NULL	lack 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Initiatives such as these are producing positive changes within healthcare organizations , but two serious barriers all but preclude improvement at the system level : a compensation process that punishes innovation and the emergence of integrated care systems that lack a common vision .
	manualset3
101915	13	401319	13	NULL	NULL	0	NULL	common vision	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Initiatives such as these are producing positive changes within healthcare organizations , but two serious barriers all but preclude improvement at the system level : a compensation process that punishes innovation and the emergence of integrated care systems that lack a common vision .
	manualset3
101916	1	401320	13	NULL	NULL	0	NULL	Injectable Poly-l-Lactic Acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Injectable Poly-l-Lactic Acid for Human Immunodeficiency Virus-Associated Facial Lipoatrophy : Cumulative Year 2 Interim Analysis of an Open-Label Study ( FACES ) .
	manualset3
101917	2	401320	13	NULL	NULL	0	NULL	Human Immunodeficiency Virus-Associated Facial Lipoatrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Injectable Poly-l-Lactic Acid for Human Immunodeficiency Virus-Associated Facial Lipoatrophy : Cumulative Year 2 Interim Analysis of an Open-Label Study ( FACES ) .
	manualset3
101918	3	401320	13	NULL	NULL	0	NULL	Cumulative Year 2 Interim Analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Injectable Poly-l-Lactic Acid for Human Immunodeficiency Virus-Associated Facial Lipoatrophy : Cumulative Year 2 Interim Analysis of an Open-Label Study ( FACES ) .
	manualset3
101919	4	401320	13	NULL	NULL	0	NULL	Open-Label Study ( FACES )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Injectable Poly-l-Lactic Acid for Human Immunodeficiency Virus-Associated Facial Lipoatrophy : Cumulative Year 2 Interim Analysis of an Open-Label Study ( FACES ) .
	manualset3
101920	1	401321	13	NULL	NULL	0	NULL	 lateral cerebral ventricle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Injected into a lateral or the third cerebral ventricle , nicotine ( 0.5 to 1 mg ) produced release of vasopressin without oxytocin .
	manualset3
101921	2	401321	13	NULL	NULL	0	NULL	third cerebral ventricle 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Injected into a lateral or the third cerebral ventricle , nicotine ( 0.5 to 1 mg ) produced release of vasopressin without oxytocin .
	manualset3
101922	3	401321	13	NULL	NULL	0	NULL	nicotine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Injected into a lateral or the third cerebral ventricle , nicotine ( 0.5 to 1 mg ) produced release of vasopressin without oxytocin .
	manualset3
101923	4	401321	13	NULL	NULL	0	NULL	0.5 to 1 mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Injected into a lateral or the third cerebral ventricle , nicotine ( 0.5 to 1 mg ) produced release of vasopressin without oxytocin .
	manualset3
101924	5	401321	13	NULL	NULL	0	NULL	release of vasopressin 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Injected into a lateral or the third cerebral ventricle , nicotine ( 0.5 to 1 mg ) produced release of vasopressin without oxytocin .
	manualset3
101925	6	401321	13	NULL	NULL	0	NULL	oxytocin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Injected into a lateral or the third cerebral ventricle , nicotine ( 0.5 to 1 mg ) produced release of vasopressin without oxytocin .
	manualset3
101926	1	401322	13	NULL	NULL	0	NULL	Injection 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Injection of a CCK-B-receptor antagonist had the opposite behavioural effect .
	manualset3
101927	2	401322	13	NULL	NULL	0	NULL	CCK-B-receptor antagonist	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Injection of a CCK-B-receptor antagonist had the opposite behavioural effect .
	manualset3
101928	3	401322	13	NULL	NULL	0	NULL	behavioural effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Injection of a CCK-B-receptor antagonist had the opposite behavioural effect .
	manualset3
101929	1	401323	13	NULL	NULL	0	NULL	Injection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Injection of antisense oligonucleotides with ability to disrupt translation of irf6 transcripts caused little or no effect on development .
	manualset3
101930	2	401323	13	NULL	NULL	0	NULL	antisense oligonucleotides	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Injection of antisense oligonucleotides with ability to disrupt translation of irf6 transcripts caused little or no effect on development .
	manualset3
101931	3	401323	13	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Injection of antisense oligonucleotides with ability to disrupt translation of irf6 transcripts caused little or no effect on development .
	manualset3
101932	4	401323	13	NULL	NULL	0	NULL	translation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Injection of antisense oligonucleotides with ability to disrupt translation of irf6 transcripts caused little or no effect on development .
	manualset3
101933	5	401323	13	NULL	NULL	0	NULL	irf6 transcripts 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Injection of antisense oligonucleotides with ability to disrupt translation of irf6 transcripts caused little or no effect on development .
	manualset3
101934	6	401323	13	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Injection of antisense oligonucleotides with ability to disrupt translation of irf6 transcripts caused little or no effect on development .
	manualset3
101935	7	401323	13	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Injection of antisense oligonucleotides with ability to disrupt translation of irf6 transcripts caused little or no effect on development .
	manualset3
101936	1	401324	13	NULL	NULL	0	NULL	Injections	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Injections of the second somatosensory area ( SmII ) and the parietal association cortex ( areas 5 and 7 ) gave moderate degrees of overlap .
	manualset3
101937	2	401324	13	NULL	NULL	0	NULL	second somatosensory area ( SmII )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Injections of the second somatosensory area ( SmII ) and the parietal association cortex ( areas 5 and 7 ) gave moderate degrees of overlap .
	manualset3
101938	3	401324	13	NULL	NULL	0	NULL	parietal association cortex ( areas 5 and 7 )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Injections of the second somatosensory area ( SmII ) and the parietal association cortex ( areas 5 and 7 ) gave moderate degrees of overlap .
	manualset3
101939	4	401324	13	NULL	NULL	0	NULL	moderate degrees	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Injections of the second somatosensory area ( SmII ) and the parietal association cortex ( areas 5 and 7 ) gave moderate degrees of overlap .
	manualset3
101940	1	401325	13	NULL	NULL	0	NULL	Injuries 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Injuries to the carpometacarpal ( CMC ) joints are uncommon injuries and isolated dislocation of these joints occurs very infrequently .
	manualset3
101941	2	401325	13	NULL	NULL	0	NULL	carpometacarpal ( CMC ) joints 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Injuries to the carpometacarpal ( CMC ) joints are uncommon injuries and isolated dislocation of these joints occurs very infrequently .
	manualset3
101942	3	401325	13	NULL	NULL	0	NULL	uncommon injuries	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Injuries to the carpometacarpal ( CMC ) joints are uncommon injuries and isolated dislocation of these joints occurs very infrequently .
	manualset3
101943	4	401325	13	NULL	NULL	0	NULL	dislocation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Injuries to the carpometacarpal ( CMC ) joints are uncommon injuries and isolated dislocation of these joints occurs very infrequently .
	manualset3
101944	5	401325	13	NULL	NULL	0	NULL	joints 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Injuries to the carpometacarpal ( CMC ) joints are uncommon injuries and isolated dislocation of these joints occurs very infrequently .
	manualset3
101945	1	401326	13	NULL	NULL	0	NULL	Injuries 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Injuries to the portal triad are uncommon , difficult to diagnose , and technically challenging .
	manualset3
101946	2	401326	13	NULL	NULL	0	NULL	portal triad	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Injuries to the portal triad are uncommon , difficult to diagnose , and technically challenging .
	manualset3
101947	1	401327	13	NULL	NULL	0	NULL	Injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury of myocardium caused by I/R includes cardiac contractile dysfunction , arrhythmias , as well as irreversible myocyte damage .
	manualset3
101948	2	401327	13	NULL	NULL	0	NULL	myocardium 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury of myocardium caused by I/R includes cardiac contractile dysfunction , arrhythmias , as well as irreversible myocyte damage .
	manualset3
101949	3	401327	13	NULL	NULL	0	NULL	I/R 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury of myocardium caused by I/R includes cardiac contractile dysfunction , arrhythmias , as well as irreversible myocyte damage .
	manualset3
101950	4	401327	13	NULL	NULL	0	NULL	cardiac contractile dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury of myocardium caused by I/R includes cardiac contractile dysfunction , arrhythmias , as well as irreversible myocyte damage .
	manualset3
101951	5	401327	13	NULL	NULL	0	NULL	arrhythmias	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury of myocardium caused by I/R includes cardiac contractile dysfunction , arrhythmias , as well as irreversible myocyte damage .
	manualset3
101952	6	401327	13	NULL	NULL	0	NULL	irreversible myocyte damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury of myocardium caused by I/R includes cardiac contractile dysfunction , arrhythmias , as well as irreversible myocyte damage .
	manualset3
101953	1	401328	13	NULL	NULL	0	NULL	Injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury to the common ( n = 19 cases ) , external ( n = 7 ) , internal carotid ( n = 5 ) , innominate ( n = 2 ) , subclavian ( n = 20 ) , vertebral ( n = 12 ) , facial ( n = 2 ) , and intercostal ( n = 2 ) arteries ; the external ( n = 36 ) , internal ( n = 65 ) , subclavian ( n = 20 ) , and innominate ( n = 4 ) veins ; the pharynx/esophagus ( n = 21 ) ; and the trachea ( n = 28 ) was considered a positive NE ( n = 167 ) .
	manualset3
101954	2	401328	13	NULL	NULL	0	NULL	common arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury to the common ( n = 19 cases ) , external ( n = 7 ) , internal carotid ( n = 5 ) , innominate ( n = 2 ) , subclavian ( n = 20 ) , vertebral ( n = 12 ) , facial ( n = 2 ) , and intercostal ( n = 2 ) arteries ; the external ( n = 36 ) , internal ( n = 65 ) , subclavian ( n = 20 ) , and innominate ( n = 4 ) veins ; the pharynx/esophagus ( n = 21 ) ; and the trachea ( n = 28 ) was considered a positive NE ( n = 167 ) .
	manualset3
101955	3	401328	13	NULL	NULL	0	NULL	n = 19 cases	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury to the common ( n = 19 cases ) , external ( n = 7 ) , internal carotid ( n = 5 ) , innominate ( n = 2 ) , subclavian ( n = 20 ) , vertebral ( n = 12 ) , facial ( n = 2 ) , and intercostal ( n = 2 ) arteries ; the external ( n = 36 ) , internal ( n = 65 ) , subclavian ( n = 20 ) , and innominate ( n = 4 ) veins ; the pharynx/esophagus ( n = 21 ) ; and the trachea ( n = 28 ) was considered a positive NE ( n = 167 ) .
	manualset3
101956	4	401328	13	NULL	NULL	0	NULL	external arteries 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury to the common ( n = 19 cases ) , external ( n = 7 ) , internal carotid ( n = 5 ) , innominate ( n = 2 ) , subclavian ( n = 20 ) , vertebral ( n = 12 ) , facial ( n = 2 ) , and intercostal ( n = 2 ) arteries ; the external ( n = 36 ) , internal ( n = 65 ) , subclavian ( n = 20 ) , and innominate ( n = 4 ) veins ; the pharynx/esophagus ( n = 21 ) ; and the trachea ( n = 28 ) was considered a positive NE ( n = 167 ) .
	manualset3
101957	5	401328	13	NULL	NULL	0	NULL	n = 7	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury to the common ( n = 19 cases ) , external ( n = 7 ) , internal carotid ( n = 5 ) , innominate ( n = 2 ) , subclavian ( n = 20 ) , vertebral ( n = 12 ) , facial ( n = 2 ) , and intercostal ( n = 2 ) arteries ; the external ( n = 36 ) , internal ( n = 65 ) , subclavian ( n = 20 ) , and innominate ( n = 4 ) veins ; the pharynx/esophagus ( n = 21 ) ; and the trachea ( n = 28 ) was considered a positive NE ( n = 167 ) .
	manualset3
101958	6	401328	13	NULL	NULL	0	NULL	internal carotid arteries 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury to the common ( n = 19 cases ) , external ( n = 7 ) , internal carotid ( n = 5 ) , innominate ( n = 2 ) , subclavian ( n = 20 ) , vertebral ( n = 12 ) , facial ( n = 2 ) , and intercostal ( n = 2 ) arteries ; the external ( n = 36 ) , internal ( n = 65 ) , subclavian ( n = 20 ) , and innominate ( n = 4 ) veins ; the pharynx/esophagus ( n = 21 ) ; and the trachea ( n = 28 ) was considered a positive NE ( n = 167 ) .
	manualset3
101959	7	401328	13	NULL	NULL	0	NULL	n = 5 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury to the common ( n = 19 cases ) , external ( n = 7 ) , internal carotid ( n = 5 ) , innominate ( n = 2 ) , subclavian ( n = 20 ) , vertebral ( n = 12 ) , facial ( n = 2 ) , and intercostal ( n = 2 ) arteries ; the external ( n = 36 ) , internal ( n = 65 ) , subclavian ( n = 20 ) , and innominate ( n = 4 ) veins ; the pharynx/esophagus ( n = 21 ) ; and the trachea ( n = 28 ) was considered a positive NE ( n = 167 ) .
	manualset3
101960	8	401328	13	NULL	NULL	0	NULL	innominate arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury to the common ( n = 19 cases ) , external ( n = 7 ) , internal carotid ( n = 5 ) , innominate ( n = 2 ) , subclavian ( n = 20 ) , vertebral ( n = 12 ) , facial ( n = 2 ) , and intercostal ( n = 2 ) arteries ; the external ( n = 36 ) , internal ( n = 65 ) , subclavian ( n = 20 ) , and innominate ( n = 4 ) veins ; the pharynx/esophagus ( n = 21 ) ; and the trachea ( n = 28 ) was considered a positive NE ( n = 167 ) .
	manualset3
101961	9	401328	13	NULL	NULL	0	NULL	n = 2 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury to the common ( n = 19 cases ) , external ( n = 7 ) , internal carotid ( n = 5 ) , innominate ( n = 2 ) , subclavian ( n = 20 ) , vertebral ( n = 12 ) , facial ( n = 2 ) , and intercostal ( n = 2 ) arteries ; the external ( n = 36 ) , internal ( n = 65 ) , subclavian ( n = 20 ) , and innominate ( n = 4 ) veins ; the pharynx/esophagus ( n = 21 ) ; and the trachea ( n = 28 ) was considered a positive NE ( n = 167 ) .
	manualset3
101962	10	401328	13	NULL	NULL	0	NULL	subclavian arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury to the common ( n = 19 cases ) , external ( n = 7 ) , internal carotid ( n = 5 ) , innominate ( n = 2 ) , subclavian ( n = 20 ) , vertebral ( n = 12 ) , facial ( n = 2 ) , and intercostal ( n = 2 ) arteries ; the external ( n = 36 ) , internal ( n = 65 ) , subclavian ( n = 20 ) , and innominate ( n = 4 ) veins ; the pharynx/esophagus ( n = 21 ) ; and the trachea ( n = 28 ) was considered a positive NE ( n = 167 ) .
	manualset3
101963	11	401328	13	NULL	NULL	0	NULL	n = 20	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury to the common ( n = 19 cases ) , external ( n = 7 ) , internal carotid ( n = 5 ) , innominate ( n = 2 ) , subclavian ( n = 20 ) , vertebral ( n = 12 ) , facial ( n = 2 ) , and intercostal ( n = 2 ) arteries ; the external ( n = 36 ) , internal ( n = 65 ) , subclavian ( n = 20 ) , and innominate ( n = 4 ) veins ; the pharynx/esophagus ( n = 21 ) ; and the trachea ( n = 28 ) was considered a positive NE ( n = 167 ) .
	manualset3
101964	12	401328	13	NULL	NULL	0	NULL	vertebral arteries 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury to the common ( n = 19 cases ) , external ( n = 7 ) , internal carotid ( n = 5 ) , innominate ( n = 2 ) , subclavian ( n = 20 ) , vertebral ( n = 12 ) , facial ( n = 2 ) , and intercostal ( n = 2 ) arteries ; the external ( n = 36 ) , internal ( n = 65 ) , subclavian ( n = 20 ) , and innominate ( n = 4 ) veins ; the pharynx/esophagus ( n = 21 ) ; and the trachea ( n = 28 ) was considered a positive NE ( n = 167 ) .
	manualset3
101965	13	401328	13	NULL	NULL	0	NULL	n = 12	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury to the common ( n = 19 cases ) , external ( n = 7 ) , internal carotid ( n = 5 ) , innominate ( n = 2 ) , subclavian ( n = 20 ) , vertebral ( n = 12 ) , facial ( n = 2 ) , and intercostal ( n = 2 ) arteries ; the external ( n = 36 ) , internal ( n = 65 ) , subclavian ( n = 20 ) , and innominate ( n = 4 ) veins ; the pharynx/esophagus ( n = 21 ) ; and the trachea ( n = 28 ) was considered a positive NE ( n = 167 ) .
	manualset3
101966	14	401328	13	NULL	NULL	0	NULL	facial arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury to the common ( n = 19 cases ) , external ( n = 7 ) , internal carotid ( n = 5 ) , innominate ( n = 2 ) , subclavian ( n = 20 ) , vertebral ( n = 12 ) , facial ( n = 2 ) , and intercostal ( n = 2 ) arteries ; the external ( n = 36 ) , internal ( n = 65 ) , subclavian ( n = 20 ) , and innominate ( n = 4 ) veins ; the pharynx/esophagus ( n = 21 ) ; and the trachea ( n = 28 ) was considered a positive NE ( n = 167 ) .
	manualset3
101967	15	401328	13	NULL	NULL	0	NULL	n = 2 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury to the common ( n = 19 cases ) , external ( n = 7 ) , internal carotid ( n = 5 ) , innominate ( n = 2 ) , subclavian ( n = 20 ) , vertebral ( n = 12 ) , facial ( n = 2 ) , and intercostal ( n = 2 ) arteries ; the external ( n = 36 ) , internal ( n = 65 ) , subclavian ( n = 20 ) , and innominate ( n = 4 ) veins ; the pharynx/esophagus ( n = 21 ) ; and the trachea ( n = 28 ) was considered a positive NE ( n = 167 ) .
	manualset3
101968	16	401328	13	NULL	NULL	0	NULL	intercostal arteries 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury to the common ( n = 19 cases ) , external ( n = 7 ) , internal carotid ( n = 5 ) , innominate ( n = 2 ) , subclavian ( n = 20 ) , vertebral ( n = 12 ) , facial ( n = 2 ) , and intercostal ( n = 2 ) arteries ; the external ( n = 36 ) , internal ( n = 65 ) , subclavian ( n = 20 ) , and innominate ( n = 4 ) veins ; the pharynx/esophagus ( n = 21 ) ; and the trachea ( n = 28 ) was considered a positive NE ( n = 167 ) .
	manualset3
101969	17	401328	13	NULL	NULL	0	NULL	n = 2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury to the common ( n = 19 cases ) , external ( n = 7 ) , internal carotid ( n = 5 ) , innominate ( n = 2 ) , subclavian ( n = 20 ) , vertebral ( n = 12 ) , facial ( n = 2 ) , and intercostal ( n = 2 ) arteries ; the external ( n = 36 ) , internal ( n = 65 ) , subclavian ( n = 20 ) , and innominate ( n = 4 ) veins ; the pharynx/esophagus ( n = 21 ) ; and the trachea ( n = 28 ) was considered a positive NE ( n = 167 ) .
	manualset3
101970	18	401328	13	NULL	NULL	0	NULL	 external veins	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury to the common ( n = 19 cases ) , external ( n = 7 ) , internal carotid ( n = 5 ) , innominate ( n = 2 ) , subclavian ( n = 20 ) , vertebral ( n = 12 ) , facial ( n = 2 ) , and intercostal ( n = 2 ) arteries ; the external ( n = 36 ) , internal ( n = 65 ) , subclavian ( n = 20 ) , and innominate ( n = 4 ) veins ; the pharynx/esophagus ( n = 21 ) ; and the trachea ( n = 28 ) was considered a positive NE ( n = 167 ) .
	manualset3
101971	19	401328	13	NULL	NULL	0	NULL	n = 36	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury to the common ( n = 19 cases ) , external ( n = 7 ) , internal carotid ( n = 5 ) , innominate ( n = 2 ) , subclavian ( n = 20 ) , vertebral ( n = 12 ) , facial ( n = 2 ) , and intercostal ( n = 2 ) arteries ; the external ( n = 36 ) , internal ( n = 65 ) , subclavian ( n = 20 ) , and innominate ( n = 4 ) veins ; the pharynx/esophagus ( n = 21 ) ; and the trachea ( n = 28 ) was considered a positive NE ( n = 167 ) .
	manualset3
101972	20	401328	13	NULL	NULL	0	NULL	internal veins	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury to the common ( n = 19 cases ) , external ( n = 7 ) , internal carotid ( n = 5 ) , innominate ( n = 2 ) , subclavian ( n = 20 ) , vertebral ( n = 12 ) , facial ( n = 2 ) , and intercostal ( n = 2 ) arteries ; the external ( n = 36 ) , internal ( n = 65 ) , subclavian ( n = 20 ) , and innominate ( n = 4 ) veins ; the pharynx/esophagus ( n = 21 ) ; and the trachea ( n = 28 ) was considered a positive NE ( n = 167 ) .
	manualset3
101973	21	401328	13	NULL	NULL	0	NULL	n = 65	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury to the common ( n = 19 cases ) , external ( n = 7 ) , internal carotid ( n = 5 ) , innominate ( n = 2 ) , subclavian ( n = 20 ) , vertebral ( n = 12 ) , facial ( n = 2 ) , and intercostal ( n = 2 ) arteries ; the external ( n = 36 ) , internal ( n = 65 ) , subclavian ( n = 20 ) , and innominate ( n = 4 ) veins ; the pharynx/esophagus ( n = 21 ) ; and the trachea ( n = 28 ) was considered a positive NE ( n = 167 ) .
	manualset3
101974	22	401328	13	NULL	NULL	0	NULL	subclavian veins 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury to the common ( n = 19 cases ) , external ( n = 7 ) , internal carotid ( n = 5 ) , innominate ( n = 2 ) , subclavian ( n = 20 ) , vertebral ( n = 12 ) , facial ( n = 2 ) , and intercostal ( n = 2 ) arteries ; the external ( n = 36 ) , internal ( n = 65 ) , subclavian ( n = 20 ) , and innominate ( n = 4 ) veins ; the pharynx/esophagus ( n = 21 ) ; and the trachea ( n = 28 ) was considered a positive NE ( n = 167 ) .
	manualset3
101975	23	401328	13	NULL	NULL	0	NULL	n = 20	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury to the common ( n = 19 cases ) , external ( n = 7 ) , internal carotid ( n = 5 ) , innominate ( n = 2 ) , subclavian ( n = 20 ) , vertebral ( n = 12 ) , facial ( n = 2 ) , and intercostal ( n = 2 ) arteries ; the external ( n = 36 ) , internal ( n = 65 ) , subclavian ( n = 20 ) , and innominate ( n = 4 ) veins ; the pharynx/esophagus ( n = 21 ) ; and the trachea ( n = 28 ) was considered a positive NE ( n = 167 ) .
	manualset3
101976	24	401328	13	NULL	NULL	0	NULL	innominate veins	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury to the common ( n = 19 cases ) , external ( n = 7 ) , internal carotid ( n = 5 ) , innominate ( n = 2 ) , subclavian ( n = 20 ) , vertebral ( n = 12 ) , facial ( n = 2 ) , and intercostal ( n = 2 ) arteries ; the external ( n = 36 ) , internal ( n = 65 ) , subclavian ( n = 20 ) , and innominate ( n = 4 ) veins ; the pharynx/esophagus ( n = 21 ) ; and the trachea ( n = 28 ) was considered a positive NE ( n = 167 ) .
	manualset3
101977	25	401328	13	NULL	NULL	0	NULL	 n = 4	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury to the common ( n = 19 cases ) , external ( n = 7 ) , internal carotid ( n = 5 ) , innominate ( n = 2 ) , subclavian ( n = 20 ) , vertebral ( n = 12 ) , facial ( n = 2 ) , and intercostal ( n = 2 ) arteries ; the external ( n = 36 ) , internal ( n = 65 ) , subclavian ( n = 20 ) , and innominate ( n = 4 ) veins ; the pharynx/esophagus ( n = 21 ) ; and the trachea ( n = 28 ) was considered a positive NE ( n = 167 ) .
	manualset3
101978	26	401328	13	NULL	NULL	0	NULL	pharynx/esophagus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury to the common ( n = 19 cases ) , external ( n = 7 ) , internal carotid ( n = 5 ) , innominate ( n = 2 ) , subclavian ( n = 20 ) , vertebral ( n = 12 ) , facial ( n = 2 ) , and intercostal ( n = 2 ) arteries ; the external ( n = 36 ) , internal ( n = 65 ) , subclavian ( n = 20 ) , and innominate ( n = 4 ) veins ; the pharynx/esophagus ( n = 21 ) ; and the trachea ( n = 28 ) was considered a positive NE ( n = 167 ) .
	manualset3
101979	27	401328	13	NULL	NULL	0	NULL	n = 21 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury to the common ( n = 19 cases ) , external ( n = 7 ) , internal carotid ( n = 5 ) , innominate ( n = 2 ) , subclavian ( n = 20 ) , vertebral ( n = 12 ) , facial ( n = 2 ) , and intercostal ( n = 2 ) arteries ; the external ( n = 36 ) , internal ( n = 65 ) , subclavian ( n = 20 ) , and innominate ( n = 4 ) veins ; the pharynx/esophagus ( n = 21 ) ; and the trachea ( n = 28 ) was considered a positive NE ( n = 167 ) .
	manualset3
101980	28	401328	13	NULL	NULL	0	NULL	trachea	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury to the common ( n = 19 cases ) , external ( n = 7 ) , internal carotid ( n = 5 ) , innominate ( n = 2 ) , subclavian ( n = 20 ) , vertebral ( n = 12 ) , facial ( n = 2 ) , and intercostal ( n = 2 ) arteries ; the external ( n = 36 ) , internal ( n = 65 ) , subclavian ( n = 20 ) , and innominate ( n = 4 ) veins ; the pharynx/esophagus ( n = 21 ) ; and the trachea ( n = 28 ) was considered a positive NE ( n = 167 ) .
	manualset3
101981	29	401328	13	NULL	NULL	0	NULL	n = 28	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury to the common ( n = 19 cases ) , external ( n = 7 ) , internal carotid ( n = 5 ) , innominate ( n = 2 ) , subclavian ( n = 20 ) , vertebral ( n = 12 ) , facial ( n = 2 ) , and intercostal ( n = 2 ) arteries ; the external ( n = 36 ) , internal ( n = 65 ) , subclavian ( n = 20 ) , and innominate ( n = 4 ) veins ; the pharynx/esophagus ( n = 21 ) ; and the trachea ( n = 28 ) was considered a positive NE ( n = 167 ) .
	manualset3
101982	30	401328	13	NULL	NULL	0	NULL	positive NE ( n = 167 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Injury to the common ( n = 19 cases ) , external ( n = 7 ) , internal carotid ( n = 5 ) , innominate ( n = 2 ) , subclavian ( n = 20 ) , vertebral ( n = 12 ) , facial ( n = 2 ) , and intercostal ( n = 2 ) arteries ; the external ( n = 36 ) , internal ( n = 65 ) , subclavian ( n = 20 ) , and innominate ( n = 4 ) veins ; the pharynx/esophagus ( n = 21 ) ; and the trachea ( n = 28 ) was considered a positive NE ( n = 167 ) .
	manualset3
101983	1	401329	13	NULL	NULL	0	NULL	Inoculation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inoculation with A. brassicicola and A. alternata as biotic stresses increased transcript levels of 12 and 5 genes in Arabidopsis plants , respectively .
	manualset3
101984	2	401329	13	NULL	NULL	0	NULL	A. brassicicola 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Inoculation with A. brassicicola and A. alternata as biotic stresses increased transcript levels of 12 and 5 genes in Arabidopsis plants , respectively .
	manualset3
101985	3	401329	13	NULL	NULL	0	NULL	 A. alternata	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Inoculation with A. brassicicola and A. alternata as biotic stresses increased transcript levels of 12 and 5 genes in Arabidopsis plants , respectively .
	manualset3
101986	4	401329	13	NULL	NULL	0	NULL	biotic stresses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inoculation with A. brassicicola and A. alternata as biotic stresses increased transcript levels of 12 and 5 genes in Arabidopsis plants , respectively .
	manualset3
101987	5	401329	13	NULL	NULL	0	NULL	 transcript levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Inoculation with A. brassicicola and A. alternata as biotic stresses increased transcript levels of 12 and 5 genes in Arabidopsis plants , respectively .
	manualset3
101988	6	401329	13	NULL	NULL	0	NULL	12 genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Inoculation with A. brassicicola and A. alternata as biotic stresses increased transcript levels of 12 and 5 genes in Arabidopsis plants , respectively .
	manualset3
101989	7	401329	13	NULL	NULL	0	NULL	5 genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Inoculation with A. brassicicola and A. alternata as biotic stresses increased transcript levels of 12 and 5 genes in Arabidopsis plants , respectively .
	manualset3
101990	8	401329	13	NULL	NULL	0	NULL	Arabidopsis plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Inoculation with A. brassicicola and A. alternata as biotic stresses increased transcript levels of 12 and 5 genes in Arabidopsis plants , respectively .
	manualset3
101991	1	401330	13	NULL	NULL	0	NULL	Inoculation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Inoculation with attenuated S. typhimurium vaccines resulted in a weak but significantly reduced colonisation by S. typhimurium .
	manualset3
101992	2	401330	13	NULL	NULL	0	NULL	S. typhimurium vaccines	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Inoculation with attenuated S. typhimurium vaccines resulted in a weak but significantly reduced colonisation by S. typhimurium .
	manualset3
101993	3	401330	13	NULL	NULL	0	NULL	colonisation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inoculation with attenuated S. typhimurium vaccines resulted in a weak but significantly reduced colonisation by S. typhimurium .
	manualset3
101994	4	401330	13	NULL	NULL	0	NULL	S. typhimurium	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Inoculation with attenuated S. typhimurium vaccines resulted in a weak but significantly reduced colonisation by S. typhimurium .
	manualset3
101995	1	401331	13	NULL	NULL	0	NULL	Inoculations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Inoculations with O Manisa or C Noville did not induce clinical disease , whereas Asia1 Shamir induced death too rapidly ( i.e. within 4 days post-inoculation ( dpi ) ) .
	manualset3
101996	2	401331	13	NULL	NULL	0	NULL	O Manisa 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Inoculations with O Manisa or C Noville did not induce clinical disease , whereas Asia1 Shamir induced death too rapidly ( i.e. within 4 days post-inoculation ( dpi ) ) .
	manualset3
101997	3	401331	13	NULL	NULL	0	NULL	 C Noville 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Inoculations with O Manisa or C Noville did not induce clinical disease , whereas Asia1 Shamir induced death too rapidly ( i.e. within 4 days post-inoculation ( dpi ) ) .
	manualset3
101998	4	401331	13	NULL	NULL	0	NULL	clinical disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Inoculations with O Manisa or C Noville did not induce clinical disease , whereas Asia1 Shamir induced death too rapidly ( i.e. within 4 days post-inoculation ( dpi ) ) .
	manualset3
101999	5	401331	13	NULL	NULL	0	NULL	 Asia1 Shamir	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Inoculations with O Manisa or C Noville did not induce clinical disease , whereas Asia1 Shamir induced death too rapidly ( i.e. within 4 days post-inoculation ( dpi ) ) .
	manualset3
102000	6	401331	13	NULL	NULL	0	NULL	death 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inoculations with O Manisa or C Noville did not induce clinical disease , whereas Asia1 Shamir induced death too rapidly ( i.e. within 4 days post-inoculation ( dpi ) ) .
	manualset3
102001	7	401331	13	NULL	NULL	0	NULL	4 days	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Inoculations with O Manisa or C Noville did not induce clinical disease , whereas Asia1 Shamir induced death too rapidly ( i.e. within 4 days post-inoculation ( dpi ) ) .
	manualset3
102002	1	401332	13	NULL	NULL	0	NULL	3-Ketovalidoxylamine A C-N lyase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	3-Ketovalidoxylamine A C-N lyase of Flavobacterium saccharophilum is a monomeric protein with a molecular weight of 36 , 000 .
	manualset3
102003	2	401332	13	NULL	NULL	0	NULL	Flavobacterium saccharophilum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	3-Ketovalidoxylamine A C-N lyase of Flavobacterium saccharophilum is a monomeric protein with a molecular weight of 36 , 000 .
	manualset3
102004	3	401332	13	NULL	NULL	0	NULL	monomeric protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	3-Ketovalidoxylamine A C-N lyase of Flavobacterium saccharophilum is a monomeric protein with a molecular weight of 36 , 000 .
	manualset3
102005	4	401332	13	NULL	NULL	0	NULL	molecular weight of 36 , 000	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	3-Ketovalidoxylamine A C-N lyase of Flavobacterium saccharophilum is a monomeric protein with a molecular weight of 36 , 000 .
	manualset3
102006	1	401333	13	NULL	NULL	0	NULL	Inositol 1 , 3 , 4 , 5-tetrakisphosphate ( IP4 ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inositol 1 , 3 , 4 , 5-tetrakisphosphate ( IP4 ) , but not inositol 4 , 5 , -bisphosphate , mimicked the effect of IP3 .
	manualset3
102007	2	401333	13	NULL	NULL	0	NULL	inositol 4 , 5 , -bisphosphate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inositol 1 , 3 , 4 , 5-tetrakisphosphate ( IP4 ) , but not inositol 4 , 5 , -bisphosphate , mimicked the effect of IP3 .
	manualset3
102008	3	401333	13	NULL	NULL	0	NULL	 effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inositol 1 , 3 , 4 , 5-tetrakisphosphate ( IP4 ) , but not inositol 4 , 5 , -bisphosphate , mimicked the effect of IP3 .
	manualset3
102009	4	401333	13	NULL	NULL	0	NULL	IP3	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inositol 1 , 3 , 4 , 5-tetrakisphosphate ( IP4 ) , but not inositol 4 , 5 , -bisphosphate , mimicked the effect of IP3 .
	manualset3
102010	1	401334	13	NULL	NULL	0	NULL	Inputs	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inputs of neuropeptide Y-and serotonin-ir fibers from the host brain to grafted SCN peptide cell clusters were variable .
	manualset3
102011	2	401334	13	NULL	NULL	NULL	NULL	neuropeptide Y fibers	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Inputs of neuropeptide Y-and serotonin-ir fibers from the host brain to grafted SCN peptide cell clusters were variable .
	manualset3
102012	3	401334	13	NULL	NULL	0	NULL	serotonin-ir fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Inputs of neuropeptide Y-and serotonin-ir fibers from the host brain to grafted SCN peptide cell clusters were variable .
	manualset3
102013	4	401334	13	NULL	NULL	0	NULL	host brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Inputs of neuropeptide Y-and serotonin-ir fibers from the host brain to grafted SCN peptide cell clusters were variable .
	manualset3
102014	5	401334	13	NULL	NULL	0	NULL	SCN peptide cell clusters	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Inputs of neuropeptide Y-and serotonin-ir fibers from the host brain to grafted SCN peptide cell clusters were variable .
	manualset3
102015	1	401335	13	NULL	NULL	0	NULL	Inservice teachers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Inservice teachers ' assessed needs in behavioral disorders , mental retardation , and learning disabilities : are they similar ?
	manualset3
102016	2	401335	13	NULL	NULL	0	NULL	needs	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inservice teachers ' assessed needs in behavioral disorders , mental retardation , and learning disabilities : are they similar ?
	manualset3
102017	3	401335	13	NULL	NULL	0	NULL	behavioral disorders 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inservice teachers ' assessed needs in behavioral disorders , mental retardation , and learning disabilities : are they similar ?
	manualset3
102018	4	401335	13	NULL	NULL	0	NULL	mental retardation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inservice teachers ' assessed needs in behavioral disorders , mental retardation , and learning disabilities : are they similar ?
	manualset3
102019	5	401335	13	NULL	NULL	0	NULL	learning disabilities 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inservice teachers ' assessed needs in behavioral disorders , mental retardation , and learning disabilities : are they similar ?
	manualset3
102020	1	401336	13	NULL	NULL	0	NULL	Insights	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Insights from genomic analyses might allow psychologists to understand , predict and modify human behavior .
	manualset3
102021	2	401336	13	NULL	NULL	0	NULL	genomic analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Insights from genomic analyses might allow psychologists to understand , predict and modify human behavior .
	manualset3
102022	3	401336	13	NULL	NULL	0	NULL	psychologists 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Insights from genomic analyses might allow psychologists to understand , predict and modify human behavior .
	manualset3
102023	4	401336	13	NULL	NULL	0	NULL	 human behavior	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Insights from genomic analyses might allow psychologists to understand , predict and modify human behavior .
	manualset3
102024	1	401337	13	NULL	NULL	0	NULL	Insomnia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Insomnia and obstructive sleep apnea ( OSA ) often coexist , but the nature of their relationship is unclear .
	manualset3
102025	2	401337	13	NULL	NULL	0	NULL	obstructive sleep apnea ( OSA )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Insomnia and obstructive sleep apnea ( OSA ) often coexist , but the nature of their relationship is unclear .
	manualset3
102026	3	401337	13	NULL	NULL	0	NULL	nature	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Insomnia and obstructive sleep apnea ( OSA ) often coexist , but the nature of their relationship is unclear .
	manualset3
102027	4	401337	13	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Insomnia and obstructive sleep apnea ( OSA ) often coexist , but the nature of their relationship is unclear .
	manualset3
102028	1	401338	13	NULL	NULL	0	NULL	Inspection disclosure systems	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Inspection disclosure systems have been developed as tools for consumers and incentives for food service operators .
	manualset3
102029	2	401338	13	NULL	NULL	0	NULL	tools	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Inspection disclosure systems have been developed as tools for consumers and incentives for food service operators .
	manualset3
102030	3	401338	13	NULL	NULL	0	NULL	consumers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Inspection disclosure systems have been developed as tools for consumers and incentives for food service operators .
	manualset3
102031	4	401338	13	NULL	NULL	0	NULL	incentives	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inspection disclosure systems have been developed as tools for consumers and incentives for food service operators .
	manualset3
102032	5	401338	13	NULL	NULL	0	NULL	food service operators	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Inspection disclosure systems have been developed as tools for consumers and incentives for food service operators .
	manualset3
102034	2	401339	13	NULL	NULL	0	NULL	 advent	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inspite of the advent of newer purine analogs , in India recombinant interferon is the only freely available first line treatment .
	manualset3
102035	3	401339	13	NULL	NULL	0	NULL	purine analogs 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inspite of the advent of newer purine analogs , in India recombinant interferon is the only freely available first line treatment .
	manualset3
102036	4	401339	13	NULL	NULL	0	NULL	India	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Inspite of the advent of newer purine analogs , in India recombinant interferon is the only freely available first line treatment .
	manualset3
102037	5	401339	13	NULL	NULL	0	NULL	recombinant interferon 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Inspite of the advent of newer purine analogs , in India recombinant interferon is the only freely available first line treatment .
	manualset3
102038	6	401339	13	NULL	NULL	0	NULL	 first line treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Inspite of the advent of newer purine analogs , in India recombinant interferon is the only freely available first line treatment .
	manualset3
102039	1	401340	13	NULL	NULL	0	NULL	plasma glucose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , plasma glucose and core temperature changes appear to be the main determinants : higher glucose was related to faster and less accurate performance , whereas core temperature rises had the opposite effect .
	manualset3
102040	2	401340	13	NULL	NULL	0	NULL	core temperature changes	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , plasma glucose and core temperature changes appear to be the main determinants : higher glucose was related to faster and less accurate performance , whereas core temperature rises had the opposite effect .
	manualset3
102041	3	401340	13	NULL	NULL	0	NULL	determinants 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , plasma glucose and core temperature changes appear to be the main determinants : higher glucose was related to faster and less accurate performance , whereas core temperature rises had the opposite effect .
	manualset3
102042	4	401340	13	NULL	NULL	0	NULL	glucose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , plasma glucose and core temperature changes appear to be the main determinants : higher glucose was related to faster and less accurate performance , whereas core temperature rises had the opposite effect .
	manualset3
102043	5	401340	13	NULL	NULL	0	NULL	performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , plasma glucose and core temperature changes appear to be the main determinants : higher glucose was related to faster and less accurate performance , whereas core temperature rises had the opposite effect .
	manualset3
102044	6	401340	13	NULL	NULL	0	NULL	core temperature	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , plasma glucose and core temperature changes appear to be the main determinants : higher glucose was related to faster and less accurate performance , whereas core temperature rises had the opposite effect .
	manualset3
102045	7	401340	13	NULL	NULL	0	NULL	opposite effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , plasma glucose and core temperature changes appear to be the main determinants : higher glucose was related to faster and less accurate performance , whereas core temperature rises had the opposite effect .
	manualset3
102046	1	401341	13	NULL	NULL	0	NULL	average number of particles 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , the average number of particles that can pass through a pore before it clogs scales with the ratio of pore to particle size .
	manualset3
102047	2	401341	13	NULL	NULL	0	NULL	pore 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , the average number of particles that can pass through a pore before it clogs scales with the ratio of pore to particle size .
	manualset3
102048	3	401341	13	NULL	NULL	0	NULL	 scales	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , the average number of particles that can pass through a pore before it clogs scales with the ratio of pore to particle size .
	manualset3
102049	4	401341	13	NULL	NULL	0	NULL	 ratio of pore to particle size	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , the average number of particles that can pass through a pore before it clogs scales with the ratio of pore to particle size .
	manualset3
102050	1	401342	13	NULL	NULL	0	NULL	surface density 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , the increased surface density of the mitochondrial cristae , which has also been previously reported in patients with uncomplicated cholelithiasis , appears as an early and constant phenomenon associated with conformational changes of this mitochondrial component .
	manualset3
102051	2	401342	13	NULL	NULL	0	NULL	 mitochondrial cristae	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , the increased surface density of the mitochondrial cristae , which has also been previously reported in patients with uncomplicated cholelithiasis , appears as an early and constant phenomenon associated with conformational changes of this mitochondrial component .
	manualset3
102052	3	401342	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , the increased surface density of the mitochondrial cristae , which has also been previously reported in patients with uncomplicated cholelithiasis , appears as an early and constant phenomenon associated with conformational changes of this mitochondrial component .
	manualset3
102053	4	401342	13	NULL	NULL	0	NULL	cholelithiasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , the increased surface density of the mitochondrial cristae , which has also been previously reported in patients with uncomplicated cholelithiasis , appears as an early and constant phenomenon associated with conformational changes of this mitochondrial component .
	manualset3
102054	5	401342	13	NULL	NULL	0	NULL	phenomenon	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , the increased surface density of the mitochondrial cristae , which has also been previously reported in patients with uncomplicated cholelithiasis , appears as an early and constant phenomenon associated with conformational changes of this mitochondrial component .
	manualset3
102055	6	401342	13	NULL	NULL	0	NULL	conformational changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , the increased surface density of the mitochondrial cristae , which has also been previously reported in patients with uncomplicated cholelithiasis , appears as an early and constant phenomenon associated with conformational changes of this mitochondrial component .
	manualset3
102056	7	401342	13	NULL	NULL	0	NULL	mitochondrial component 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , the increased surface density of the mitochondrial cristae , which has also been previously reported in patients with uncomplicated cholelithiasis , appears as an early and constant phenomenon associated with conformational changes of this mitochondrial component .
	manualset3
102057	1	401343	13	NULL	NULL	0	NULL	molybdenum center	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , the molybdenum center of XOR is posttranslationally inactivated by oxygen metabolites in `` normal '' ( 21 % O2 ) cell culture atmosphere .
	manualset3
102058	2	401343	13	NULL	NULL	0	NULL	 XOR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , the molybdenum center of XOR is posttranslationally inactivated by oxygen metabolites in `` normal '' ( 21 % O2 ) cell culture atmosphere .
	manualset3
102059	3	401343	13	NULL	NULL	0	NULL	oxygen metabolites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , the molybdenum center of XOR is posttranslationally inactivated by oxygen metabolites in `` normal '' ( 21 % O2 ) cell culture atmosphere .
	manualset3
102060	4	401343	13	NULL	NULL	0	NULL	21 % O2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , the molybdenum center of XOR is posttranslationally inactivated by oxygen metabolites in `` normal '' ( 21 % O2 ) cell culture atmosphere .
	manualset3
102061	5	401343	13	NULL	NULL	0	NULL	 cell culture atmosphere	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , the molybdenum center of XOR is posttranslationally inactivated by oxygen metabolites in `` normal '' ( 21 % O2 ) cell culture atmosphere .
	manualset3
102062	1	401344	13	NULL	NULL	0	NULL	change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , there was almost no change in I11 while I10 decreased by 30 % .
	manualset3
102063	2	401344	13	NULL	NULL	0	NULL	I11	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , there was almost no change in I11 while I10 decreased by 30 % .
	manualset3
102064	3	401344	13	NULL	NULL	0	NULL	I10 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , there was almost no change in I11 while I10 decreased by 30 % .
	manualset3
102065	4	401344	13	NULL	NULL	0	NULL	30 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , there was almost no change in I11 while I10 decreased by 30 % .
	manualset3
102066	1	401345	13	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , we hypothesize that the number of fungal serine proteases in a species is related to the use of the animal as a food source , whether it is dead or alive .
	manualset3
102067	2	401345	13	NULL	NULL	0	NULL	fungal serine proteases 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , we hypothesize that the number of fungal serine proteases in a species is related to the use of the animal as a food source , whether it is dead or alive .
	manualset3
102068	3	401345	13	NULL	NULL	0	NULL	species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , we hypothesize that the number of fungal serine proteases in a species is related to the use of the animal as a food source , whether it is dead or alive .
	manualset3
102069	4	401345	13	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , we hypothesize that the number of fungal serine proteases in a species is related to the use of the animal as a food source , whether it is dead or alive .
	manualset3
102070	5	401345	13	NULL	NULL	0	NULL	animal 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , we hypothesize that the number of fungal serine proteases in a species is related to the use of the animal as a food source , whether it is dead or alive .
	manualset3
102071	6	401345	13	NULL	NULL	0	NULL	food source	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , we hypothesize that the number of fungal serine proteases in a species is related to the use of the animal as a food source , whether it is dead or alive .
	manualset3
102072	1	401346	13	NULL	NULL	0	NULL	 increase in quantum yield	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , we observe a step-like increase in quantum yield for larger photon energies that is characteristic of carrier multiplication .
	manualset3
102073	2	401346	13	NULL	NULL	0	NULL	larger photon energies 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , we observe a step-like increase in quantum yield for larger photon energies that is characteristic of carrier multiplication .
	manualset3
102074	3	401346	13	NULL	NULL	0	NULL	carrier multiplication	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead , we observe a step-like increase in quantum yield for larger photon energies that is characteristic of carrier multiplication .
	manualset3
102075	1	401347	13	NULL	NULL	0	NULL	130 kDa protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead of an expected 130 kDa protein , two proteins of 40 and 90 kDa were identified as the gene product of ORF6 which might arise from cotranslational cleavage ( 18 ) .
	manualset3
102076	2	401347	13	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead of an expected 130 kDa protein , two proteins of 40 and 90 kDa were identified as the gene product of ORF6 which might arise from cotranslational cleavage ( 18 ) .
	manualset3
102077	3	401347	13	NULL	NULL	0	NULL	protein of 40 kDa 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead of an expected 130 kDa protein , two proteins of 40 and 90 kDa were identified as the gene product of ORF6 which might arise from cotranslational cleavage ( 18 ) .
	manualset3
102078	4	401347	13	NULL	NULL	0	NULL	protein of 90 kDa	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead of an expected 130 kDa protein , two proteins of 40 and 90 kDa were identified as the gene product of ORF6 which might arise from cotranslational cleavage ( 18 ) .
	manualset3
102079	5	401347	13	NULL	NULL	0	NULL	 gene product	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead of an expected 130 kDa protein , two proteins of 40 and 90 kDa were identified as the gene product of ORF6 which might arise from cotranslational cleavage ( 18 ) .
	manualset3
102080	6	401347	13	NULL	NULL	0	NULL	ORF6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead of an expected 130 kDa protein , two proteins of 40 and 90 kDa were identified as the gene product of ORF6 which might arise from cotranslational cleavage ( 18 ) .
	manualset3
102081	7	401347	13	NULL	NULL	0	NULL	 cotranslational cleavage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead of an expected 130 kDa protein , two proteins of 40 and 90 kDa were identified as the gene product of ORF6 which might arise from cotranslational cleavage ( 18 ) .
	manualset3
102082	1	401348	13	NULL	NULL	0	NULL	sheathing mycorrhizal fungi	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead of classifying sheathing mycorrhizal fungi by referring to the temporal stage of woodland development , it now seems more meaningful to judge them by their abilities to colonize roots in soils with or without accumulations of different types of litter .
	manualset3
102083	2	401348	13	NULL	NULL	0	NULL	temporal stage	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead of classifying sheathing mycorrhizal fungi by referring to the temporal stage of woodland development , it now seems more meaningful to judge them by their abilities to colonize roots in soils with or without accumulations of different types of litter .
	manualset3
102084	3	401348	13	NULL	NULL	0	NULL	woodland	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead of classifying sheathing mycorrhizal fungi by referring to the temporal stage of woodland development , it now seems more meaningful to judge them by their abilities to colonize roots in soils with or without accumulations of different types of litter .
	manualset3
102085	4	401348	13	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead of classifying sheathing mycorrhizal fungi by referring to the temporal stage of woodland development , it now seems more meaningful to judge them by their abilities to colonize roots in soils with or without accumulations of different types of litter .
	manualset3
102086	5	401348	13	NULL	NULL	0	NULL	abilities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead of classifying sheathing mycorrhizal fungi by referring to the temporal stage of woodland development , it now seems more meaningful to judge them by their abilities to colonize roots in soils with or without accumulations of different types of litter .
	manualset3
102087	6	401348	13	NULL	NULL	0	NULL	colonize	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead of classifying sheathing mycorrhizal fungi by referring to the temporal stage of woodland development , it now seems more meaningful to judge them by their abilities to colonize roots in soils with or without accumulations of different types of litter .
	manualset3
102088	7	401348	13	NULL	NULL	0	NULL	roots 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead of classifying sheathing mycorrhizal fungi by referring to the temporal stage of woodland development , it now seems more meaningful to judge them by their abilities to colonize roots in soils with or without accumulations of different types of litter .
	manualset3
102089	8	401348	13	NULL	NULL	0	NULL	soils	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead of classifying sheathing mycorrhizal fungi by referring to the temporal stage of woodland development , it now seems more meaningful to judge them by their abilities to colonize roots in soils with or without accumulations of different types of litter .
	manualset3
102090	9	401348	13	NULL	NULL	0	NULL	accumulations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead of classifying sheathing mycorrhizal fungi by referring to the temporal stage of woodland development , it now seems more meaningful to judge them by their abilities to colonize roots in soils with or without accumulations of different types of litter .
	manualset3
102091	10	401348	13	NULL	NULL	0	NULL	different types of litter	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead of classifying sheathing mycorrhizal fungi by referring to the temporal stage of woodland development , it now seems more meaningful to judge them by their abilities to colonize roots in soils with or without accumulations of different types of litter .
	manualset3
102092	1	401349	13	NULL	NULL	NULL	NULL	paramagnetic centres 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Instead of paramagnetic centres , which are native in biological systems , very often the molecules with a free radical are incorporated into the system -- spin labels or spin probes .
	manualset3
102093	2	401349	13	NULL	NULL	0	NULL	biological systems	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead of paramagnetic centres , which are native in biological systems , very often the molecules with a free radical are incorporated into the system -- spin labels or spin probes .
	manualset3
102094	3	401349	13	NULL	NULL	0	NULL	molecules 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead of paramagnetic centres , which are native in biological systems , very often the molecules with a free radical are incorporated into the system -- spin labels or spin probes .
	manualset3
102095	4	401349	13	NULL	NULL	0	NULL	free radical	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead of paramagnetic centres , which are native in biological systems , very often the molecules with a free radical are incorporated into the system -- spin labels or spin probes .
	manualset3
102096	5	401349	13	NULL	NULL	0	NULL	system 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead of paramagnetic centres , which are native in biological systems , very often the molecules with a free radical are incorporated into the system -- spin labels or spin probes .
	manualset3
102097	6	401349	13	NULL	NULL	NULL	NULL	spin labels	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Instead of paramagnetic centres , which are native in biological systems , very often the molecules with a free radical are incorporated into the system -- spin labels or spin probes .
	manualset3
102098	7	401349	13	NULL	NULL	0	NULL	spin probes	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Instead of paramagnetic centres , which are native in biological systems , very often the molecules with a free radical are incorporated into the system -- spin labels or spin probes .
	manualset3
102099	1	401350	13	NULL	NULL	0	NULL	H + - linked porters	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	3 ) H + - linked porters such as a H + - driven amino acid carrier and a Na + - H + antiporter were characterized .
	manualset3
102100	2	401350	13	NULL	NULL	0	NULL	H + - driven amino acid carrier	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	3 ) H + - linked porters such as a H + - driven amino acid carrier and a Na + - H + antiporter were characterized .
	manualset3
102101	3	401350	13	NULL	NULL	0	NULL	Na + - H + antiporter	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	3 ) H + - linked porters such as a H + - driven amino acid carrier and a Na + - H + antiporter were characterized .
	manualset3
102102	1	401351	13	NULL	NULL	0	NULL	Instruction effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Instruction effects in implicit artificial grammar learning : a preference for grammaticality .
	manualset3
102103	2	401351	13	NULL	NULL	0	NULL	artificial grammar learning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Instruction effects in implicit artificial grammar learning : a preference for grammaticality .
	manualset3
102104	3	401351	13	NULL	NULL	0	NULL	preference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Instruction effects in implicit artificial grammar learning : a preference for grammaticality .
	manualset3
102105	1	401352	13	NULL	NULL	0	NULL	Instrumental methods	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Instrumental methods are then discussed , from the simple dedicated compressor to the stereotactic techniques and , finally , the role of ultrasonography both in preoperative localization and in cytologic biopsy .
	manualset3
102106	2	401352	13	NULL	NULL	0	NULL	compressor	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Instrumental methods are then discussed , from the simple dedicated compressor to the stereotactic techniques and , finally , the role of ultrasonography both in preoperative localization and in cytologic biopsy .
	manualset3
102107	3	401352	13	NULL	NULL	0	NULL	stereotactic techniques	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Instrumental methods are then discussed , from the simple dedicated compressor to the stereotactic techniques and , finally , the role of ultrasonography both in preoperative localization and in cytologic biopsy .
	manualset3
102108	4	401352	13	NULL	NULL	0	NULL	role 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Instrumental methods are then discussed , from the simple dedicated compressor to the stereotactic techniques and , finally , the role of ultrasonography both in preoperative localization and in cytologic biopsy .
	manualset3
102109	5	401352	13	NULL	NULL	0	NULL	ultrasonography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Instrumental methods are then discussed , from the simple dedicated compressor to the stereotactic techniques and , finally , the role of ultrasonography both in preoperative localization and in cytologic biopsy .
	manualset3
102110	6	401352	13	NULL	NULL	0	NULL	preoperative localization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Instrumental methods are then discussed , from the simple dedicated compressor to the stereotactic techniques and , finally , the role of ultrasonography both in preoperative localization and in cytologic biopsy .
	manualset3
102111	7	401352	13	NULL	NULL	0	NULL	cytologic biopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Instrumental methods are then discussed , from the simple dedicated compressor to the stereotactic techniques and , finally , the role of ultrasonography both in preoperative localization and in cytologic biopsy .
	manualset3
102112	1	401353	13	NULL	NULL	0	NULL	Insulin-dependent diabetes mellitus ( IDDM ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-dependent diabetes mellitus ( IDDM ) HLA class II DRB1-DQA1-DQB1 data from four populations ( Norwegian , Sardinian , Mexican American , and Taiwanese ) have been analyzed to detect the amino acids involved in the disease process .
	manualset3
102113	2	401353	13	NULL	NULL	0	NULL	HLA class II DRB1-DQA1-DQB1 data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-dependent diabetes mellitus ( IDDM ) HLA class II DRB1-DQA1-DQB1 data from four populations ( Norwegian , Sardinian , Mexican American , and Taiwanese ) have been analyzed to detect the amino acids involved in the disease process .
	manualset3
102114	3	401353	13	NULL	NULL	0	NULL	four populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-dependent diabetes mellitus ( IDDM ) HLA class II DRB1-DQA1-DQB1 data from four populations ( Norwegian , Sardinian , Mexican American , and Taiwanese ) have been analyzed to detect the amino acids involved in the disease process .
	manualset3
102115	4	401353	13	NULL	NULL	0	NULL	Norwegian 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-dependent diabetes mellitus ( IDDM ) HLA class II DRB1-DQA1-DQB1 data from four populations ( Norwegian , Sardinian , Mexican American , and Taiwanese ) have been analyzed to detect the amino acids involved in the disease process .
	manualset3
102116	5	401353	13	NULL	NULL	0	NULL	Sardinian	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-dependent diabetes mellitus ( IDDM ) HLA class II DRB1-DQA1-DQB1 data from four populations ( Norwegian , Sardinian , Mexican American , and Taiwanese ) have been analyzed to detect the amino acids involved in the disease process .
	manualset3
102117	6	401353	13	NULL	NULL	0	NULL	Mexican American	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-dependent diabetes mellitus ( IDDM ) HLA class II DRB1-DQA1-DQB1 data from four populations ( Norwegian , Sardinian , Mexican American , and Taiwanese ) have been analyzed to detect the amino acids involved in the disease process .
	manualset3
102118	7	401353	13	NULL	NULL	0	NULL	Taiwanese	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-dependent diabetes mellitus ( IDDM ) HLA class II DRB1-DQA1-DQB1 data from four populations ( Norwegian , Sardinian , Mexican American , and Taiwanese ) have been analyzed to detect the amino acids involved in the disease process .
	manualset3
102119	8	401353	13	NULL	NULL	NULL	NULL	amino acids	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Insulin-dependent diabetes mellitus ( IDDM ) HLA class II DRB1-DQA1-DQB1 data from four populations ( Norwegian , Sardinian , Mexican American , and Taiwanese ) have been analyzed to detect the amino acids involved in the disease process .
	manualset3
102120	9	401353	13	NULL	NULL	0	NULL	 disease process 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-dependent diabetes mellitus ( IDDM ) HLA class II DRB1-DQA1-DQB1 data from four populations ( Norwegian , Sardinian , Mexican American , and Taiwanese ) have been analyzed to detect the amino acids involved in the disease process .
	manualset3
102121	1	401354	13	NULL	NULL	0	NULL	Insulin-induced phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-induced phosphorylation and activation of cyclic nucleotide phosphodiesterase 3B by the serine-threonine kinase Akt .
	manualset3
102122	2	401354	13	NULL	NULL	0	NULL	Insulin-induced activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-induced phosphorylation and activation of cyclic nucleotide phosphodiesterase 3B by the serine-threonine kinase Akt .
	manualset3
102123	3	401354	13	NULL	NULL	0	NULL	cyclic nucleotide phosphodiesterase 3B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-induced phosphorylation and activation of cyclic nucleotide phosphodiesterase 3B by the serine-threonine kinase Akt .
	manualset3
102124	4	401354	13	NULL	NULL	0	NULL	serine-threonine kinase Akt	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-induced phosphorylation and activation of cyclic nucleotide phosphodiesterase 3B by the serine-threonine kinase Akt .
	manualset3
102125	1	401355	13	NULL	NULL	0	NULL	Insulin-like Growth Factor Binding Protein-3 ( IGFBP3 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-like Growth Factor Binding Protein-3 ( IGFBP3 ) is a high-affinity binding protein shown to regulate cell growth , differentiation , and apoptosis in a variety of cellular systems .
	manualset3
102126	2	401355	13	NULL	NULL	0	NULL	high-affinity binding protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-like Growth Factor Binding Protein-3 ( IGFBP3 ) is a high-affinity binding protein shown to regulate cell growth , differentiation , and apoptosis in a variety of cellular systems .
	manualset3
102127	3	401355	13	NULL	NULL	0	NULL	 cell growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-like Growth Factor Binding Protein-3 ( IGFBP3 ) is a high-affinity binding protein shown to regulate cell growth , differentiation , and apoptosis in a variety of cellular systems .
	manualset3
102128	4	401355	13	NULL	NULL	0	NULL	differentiation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-like Growth Factor Binding Protein-3 ( IGFBP3 ) is a high-affinity binding protein shown to regulate cell growth , differentiation , and apoptosis in a variety of cellular systems .
	manualset3
102129	5	401355	13	NULL	NULL	0	NULL	apoptosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-like Growth Factor Binding Protein-3 ( IGFBP3 ) is a high-affinity binding protein shown to regulate cell growth , differentiation , and apoptosis in a variety of cellular systems .
	manualset3
102130	6	401355	13	NULL	NULL	0	NULL	variety of cellular systems	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-like Growth Factor Binding Protein-3 ( IGFBP3 ) is a high-affinity binding protein shown to regulate cell growth , differentiation , and apoptosis in a variety of cellular systems .
	manualset3
102131	1	401356	13	NULL	NULL	0	NULL	Insulin-like growth factor binding protein-3 ( IGFBP-3 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-like growth factor binding protein-3 ( IGFBP-3 ) is a member of the IGFBP family , which regulates the mitogenic and antiapoptotic effects of insulin-like growth factors .
	manualset3
102132	2	401356	13	NULL	NULL	0	NULL	member	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-like growth factor binding protein-3 ( IGFBP-3 ) is a member of the IGFBP family , which regulates the mitogenic and antiapoptotic effects of insulin-like growth factors .
	manualset3
102133	3	401356	13	NULL	NULL	0	NULL	IGFBP family 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-like growth factor binding protein-3 ( IGFBP-3 ) is a member of the IGFBP family , which regulates the mitogenic and antiapoptotic effects of insulin-like growth factors .
	manualset3
102134	4	401356	13	NULL	NULL	0	NULL	mitogenic effects 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-like growth factor binding protein-3 ( IGFBP-3 ) is a member of the IGFBP family , which regulates the mitogenic and antiapoptotic effects of insulin-like growth factors .
	manualset3
102135	5	401356	13	NULL	NULL	0	NULL	antiapoptotic effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-like growth factor binding protein-3 ( IGFBP-3 ) is a member of the IGFBP family , which regulates the mitogenic and antiapoptotic effects of insulin-like growth factors .
	manualset3
102136	6	401356	13	NULL	NULL	0	NULL	insulin-like growth factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-like growth factor binding protein-3 ( IGFBP-3 ) is a member of the IGFBP family , which regulates the mitogenic and antiapoptotic effects of insulin-like growth factors .
	manualset3
102137	1	401357	13	NULL	NULL	NULL	NULL	Insulin 's 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Insulin 's effect on glucose transport activity and the subcellular distribution of glucose transporters have been examined in isolated human abdominal adipose cells , by measuring 3-O-methylglucose transport and specific D-glucose-inhibitable cytochalasin B binding to plasma membranes and low-density microsomes , respectively .
	manualset3
102138	2	401357	13	NULL	NULL	0	NULL	 effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin 's effect on glucose transport activity and the subcellular distribution of glucose transporters have been examined in isolated human abdominal adipose cells , by measuring 3-O-methylglucose transport and specific D-glucose-inhibitable cytochalasin B binding to plasma membranes and low-density microsomes , respectively .
	manualset3
102139	3	401357	13	NULL	NULL	0	NULL	glucose transport activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin 's effect on glucose transport activity and the subcellular distribution of glucose transporters have been examined in isolated human abdominal adipose cells , by measuring 3-O-methylglucose transport and specific D-glucose-inhibitable cytochalasin B binding to plasma membranes and low-density microsomes , respectively .
	manualset3
102140	4	401357	13	NULL	NULL	0	NULL	subcellular distribution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin 's effect on glucose transport activity and the subcellular distribution of glucose transporters have been examined in isolated human abdominal adipose cells , by measuring 3-O-methylglucose transport and specific D-glucose-inhibitable cytochalasin B binding to plasma membranes and low-density microsomes , respectively .
	manualset3
102141	5	401357	13	NULL	NULL	0	NULL	glucose transporters	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin 's effect on glucose transport activity and the subcellular distribution of glucose transporters have been examined in isolated human abdominal adipose cells , by measuring 3-O-methylglucose transport and specific D-glucose-inhibitable cytochalasin B binding to plasma membranes and low-density microsomes , respectively .
	manualset3
102142	6	401357	13	NULL	NULL	0	NULL	human abdominal adipose cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin 's effect on glucose transport activity and the subcellular distribution of glucose transporters have been examined in isolated human abdominal adipose cells , by measuring 3-O-methylglucose transport and specific D-glucose-inhibitable cytochalasin B binding to plasma membranes and low-density microsomes , respectively .
	manualset3
102143	7	401357	13	NULL	NULL	0	NULL	3-O-methylglucose transport	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin 's effect on glucose transport activity and the subcellular distribution of glucose transporters have been examined in isolated human abdominal adipose cells , by measuring 3-O-methylglucose transport and specific D-glucose-inhibitable cytochalasin B binding to plasma membranes and low-density microsomes , respectively .
	manualset3
102144	8	401357	13	NULL	NULL	0	NULL	specific D-glucose-inhibitable cytochalasin B binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin 's effect on glucose transport activity and the subcellular distribution of glucose transporters have been examined in isolated human abdominal adipose cells , by measuring 3-O-methylglucose transport and specific D-glucose-inhibitable cytochalasin B binding to plasma membranes and low-density microsomes , respectively .
	manualset3
102145	9	401357	13	NULL	NULL	0	NULL	plasma membranes 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin 's effect on glucose transport activity and the subcellular distribution of glucose transporters have been examined in isolated human abdominal adipose cells , by measuring 3-O-methylglucose transport and specific D-glucose-inhibitable cytochalasin B binding to plasma membranes and low-density microsomes , respectively .
	manualset3
102146	10	401357	13	NULL	NULL	0	NULL	low-density microsomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin 's effect on glucose transport activity and the subcellular distribution of glucose transporters have been examined in isolated human abdominal adipose cells , by measuring 3-O-methylglucose transport and specific D-glucose-inhibitable cytochalasin B binding to plasma membranes and low-density microsomes , respectively .
	manualset3
102147	1	401358	13	NULL	NULL	0	NULL	Insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin , in conjunction with glucose and amino acids , significantly stimulated glucose disposal ( P & lt ; 0.05 ) under all conditions .
	manualset3
102148	2	401358	13	NULL	NULL	0	NULL	conjunction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin , in conjunction with glucose and amino acids , significantly stimulated glucose disposal ( P & lt ; 0.05 ) under all conditions .
	manualset3
102149	3	401358	13	NULL	NULL	0	NULL	 glucose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin , in conjunction with glucose and amino acids , significantly stimulated glucose disposal ( P & lt ; 0.05 ) under all conditions .
	manualset3
102150	4	401358	13	NULL	NULL	0	NULL	amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin , in conjunction with glucose and amino acids , significantly stimulated glucose disposal ( P & lt ; 0.05 ) under all conditions .
	manualset3
102151	5	401358	13	NULL	NULL	0	NULL	glucose disposal 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin , in conjunction with glucose and amino acids , significantly stimulated glucose disposal ( P & lt ; 0.05 ) under all conditions .
	manualset3
102152	6	401358	13	NULL	NULL	0	NULL	P & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin , in conjunction with glucose and amino acids , significantly stimulated glucose disposal ( P & lt ; 0.05 ) under all conditions .
	manualset3
102153	7	401358	13	NULL	NULL	0	NULL	conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin , in conjunction with glucose and amino acids , significantly stimulated glucose disposal ( P & lt ; 0.05 ) under all conditions .
	manualset3
102154	1	401359	13	NULL	NULL	0	NULL	Polyamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	3 ) Polyamine and Zn2 + did not activate or inhibit directly the activity of phosphofructokinase and pyruvate kinase .
	manualset3
102155	2	401359	13	NULL	NULL	0	NULL	 Zn2 + 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	3 ) Polyamine and Zn2 + did not activate or inhibit directly the activity of phosphofructokinase and pyruvate kinase .
	manualset3
102156	3	401359	13	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	3 ) Polyamine and Zn2 + did not activate or inhibit directly the activity of phosphofructokinase and pyruvate kinase .
	manualset3
102157	4	401359	13	NULL	NULL	0	NULL	phosphofructokinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	3 ) Polyamine and Zn2 + did not activate or inhibit directly the activity of phosphofructokinase and pyruvate kinase .
	manualset3
102158	5	401359	13	NULL	NULL	0	NULL	pyruvate kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	3 ) Polyamine and Zn2 + did not activate or inhibit directly the activity of phosphofructokinase and pyruvate kinase .
	manualset3
102159	1	401360	13	NULL	NULL	0	NULL	Insulin binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin binding to circulating monocytes was studied in 22 normal volunteers before and 1 , 3 and 5 h after a 1400 Kcal meal .
	manualset3
102160	2	401360	13	NULL	NULL	0	NULL	circulating monocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin binding to circulating monocytes was studied in 22 normal volunteers before and 1 , 3 and 5 h after a 1400 Kcal meal .
	manualset3
102161	3	401360	13	NULL	NULL	0	NULL	22 normal volunteers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin binding to circulating monocytes was studied in 22 normal volunteers before and 1 , 3 and 5 h after a 1400 Kcal meal .
	manualset3
102162	4	401360	13	NULL	NULL	NULL	NULL	1 h	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Insulin binding to circulating monocytes was studied in 22 normal volunteers before and 1 , 3 and 5 h after a 1400 Kcal meal .
	manualset3
102163	5	401360	13	NULL	NULL	NULL	NULL	3 h	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Insulin binding to circulating monocytes was studied in 22 normal volunteers before and 1 , 3 and 5 h after a 1400 Kcal meal .
	manualset3
102164	6	401360	13	NULL	NULL	0	NULL	5 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin binding to circulating monocytes was studied in 22 normal volunteers before and 1 , 3 and 5 h after a 1400 Kcal meal .
	manualset3
102165	7	401360	13	NULL	NULL	0	NULL	1400 Kcal 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin binding to circulating monocytes was studied in 22 normal volunteers before and 1 , 3 and 5 h after a 1400 Kcal meal .
	manualset3
102166	8	401360	13	NULL	NULL	0	NULL	meal	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin binding to circulating monocytes was studied in 22 normal volunteers before and 1 , 3 and 5 h after a 1400 Kcal meal .
	manualset3
102167	1	401361	13	NULL	NULL	0	NULL	Insulin binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin binding to intact cells and to a partially purified insulin receptor preparation was radically decreased to 20 % and 18 % of the control values , respectively .
	manualset3
102168	2	401361	13	NULL	NULL	0	NULL	intact cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin binding to intact cells and to a partially purified insulin receptor preparation was radically decreased to 20 % and 18 % of the control values , respectively .
	manualset3
102169	3	401361	13	NULL	NULL	0	NULL	insulin receptor preparation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin binding to intact cells and to a partially purified insulin receptor preparation was radically decreased to 20 % and 18 % of the control values , respectively .
	manualset3
102170	4	401361	13	NULL	NULL	NULL	NULL	 20 % of the control values	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Insulin binding to intact cells and to a partially purified insulin receptor preparation was radically decreased to 20 % and 18 % of the control values , respectively .
	manualset3
102171	5	401361	13	NULL	NULL	0	NULL	18 % of the control values	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin binding to intact cells and to a partially purified insulin receptor preparation was radically decreased to 20 % and 18 % of the control values , respectively .
	manualset3
102172	1	401362	13	NULL	NULL	0	NULL	Insulin delivery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin delivery during surgery in the diabetic patient .
	manualset3
102173	2	401362	13	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin delivery during surgery in the diabetic patient .
	manualset3
102174	3	401362	13	NULL	NULL	0	NULL	diabetic patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin delivery during surgery in the diabetic patient .
	manualset3
102175	1	401363	13	NULL	NULL	0	NULL	Insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin regulation of glucose-6-phosphate dehydrogenase gene expression is rapamycin-sensitive and requires phosphatidylinositol 3-kinase .
	manualset3
102176	2	401363	13	NULL	NULL	0	NULL	regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin regulation of glucose-6-phosphate dehydrogenase gene expression is rapamycin-sensitive and requires phosphatidylinositol 3-kinase .
	manualset3
102177	3	401363	13	NULL	NULL	0	NULL	 glucose-6-phosphate dehydrogenase gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin regulation of glucose-6-phosphate dehydrogenase gene expression is rapamycin-sensitive and requires phosphatidylinositol 3-kinase .
	manualset3
102178	4	401363	13	NULL	NULL	0	NULL	phosphatidylinositol 3-kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin regulation of glucose-6-phosphate dehydrogenase gene expression is rapamycin-sensitive and requires phosphatidylinositol 3-kinase .
	manualset3
102179	1	401364	13	NULL	NULL	0	NULL	Insulin resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin resistance and hyperinsulinemia appear to be almost universal features of the polycystic ovary syndrome .
	manualset3
102180	2	401364	13	NULL	NULL	0	NULL	hyperinsulinemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin resistance and hyperinsulinemia appear to be almost universal features of the polycystic ovary syndrome .
	manualset3
102181	3	401364	13	NULL	NULL	0	NULL	features	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin resistance and hyperinsulinemia appear to be almost universal features of the polycystic ovary syndrome .
	manualset3
102182	4	401364	13	NULL	NULL	0	NULL	polycystic ovary syndrome 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin resistance and hyperinsulinemia appear to be almost universal features of the polycystic ovary syndrome .
	manualset3
102183	1	401365	13	NULL	NULL	0	NULL	Insulin resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin resistance was presumed to develop in normal glucose tolerance subjects with hyperinsulinemia .
	manualset3
102184	2	401365	13	NULL	NULL	0	NULL	glucose tolerance subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin resistance was presumed to develop in normal glucose tolerance subjects with hyperinsulinemia .
	manualset3
102185	3	401365	13	NULL	NULL	0	NULL	hyperinsulinemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin resistance was presumed to develop in normal glucose tolerance subjects with hyperinsulinemia .
	manualset3
102186	1	401366	13	NULL	NULL	0	NULL	Insulin secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin secretion and hepatic insulin clearance as determinants of hyperinsulinemia in normotolerant grossly obese adolescents .
	manualset3
102187	2	401366	13	NULL	NULL	0	NULL	hepatic insulin clearance	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin secretion and hepatic insulin clearance as determinants of hyperinsulinemia in normotolerant grossly obese adolescents .
	manualset3
102188	3	401366	13	NULL	NULL	0	NULL	determinants 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin secretion and hepatic insulin clearance as determinants of hyperinsulinemia in normotolerant grossly obese adolescents .
	manualset3
102189	4	401366	13	NULL	NULL	0	NULL	hyperinsulinemia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin secretion and hepatic insulin clearance as determinants of hyperinsulinemia in normotolerant grossly obese adolescents .
	manualset3
102190	5	401366	13	NULL	NULL	NULL	NULL	normotolerant grossly obese adolescents	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Insulin secretion and hepatic insulin clearance as determinants of hyperinsulinemia in normotolerant grossly obese adolescents .
	manualset3
102191	1	401367	13	NULL	NULL	0	NULL	3 T	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	3 T is superior to most advanced imaging techniques including diffusion , diffusion tensor imaging , perfusion , spectroscopy and functional MR imaging .
	manualset3
102192	2	401367	13	NULL	NULL	0	NULL	 imaging techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	3 T is superior to most advanced imaging techniques including diffusion , diffusion tensor imaging , perfusion , spectroscopy and functional MR imaging .
	manualset3
102193	3	401367	13	NULL	NULL	0	NULL	diffusion	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	3 T is superior to most advanced imaging techniques including diffusion , diffusion tensor imaging , perfusion , spectroscopy and functional MR imaging .
	manualset3
102194	4	401367	13	NULL	NULL	0	NULL	diffusion tensor imaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	3 T is superior to most advanced imaging techniques including diffusion , diffusion tensor imaging , perfusion , spectroscopy and functional MR imaging .
	manualset3
102195	5	401367	13	NULL	NULL	0	NULL	perfusion	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	3 T is superior to most advanced imaging techniques including diffusion , diffusion tensor imaging , perfusion , spectroscopy and functional MR imaging .
	manualset3
102196	6	401367	13	NULL	NULL	0	NULL	spectroscopy 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	3 T is superior to most advanced imaging techniques including diffusion , diffusion tensor imaging , perfusion , spectroscopy and functional MR imaging .
	manualset3
102197	7	401367	13	NULL	NULL	0	NULL	functional MR imaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	3 T is superior to most advanced imaging techniques including diffusion , diffusion tensor imaging , perfusion , spectroscopy and functional MR imaging .
	manualset3
102198	1	401368	13	NULL	NULL	0	NULL	Insulin secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin secretion from the pancreatic - cell is controlled by changes in membrane potential and intracellular Ca ( 2 + ) .
	manualset3
102199	2	401368	13	NULL	NULL	0	NULL	pancreatic - cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin secretion from the pancreatic - cell is controlled by changes in membrane potential and intracellular Ca ( 2 + ) .
	manualset3
102200	3	401368	13	NULL	NULL	0	NULL	 changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin secretion from the pancreatic - cell is controlled by changes in membrane potential and intracellular Ca ( 2 + ) .
	manualset3
102201	4	401368	13	NULL	NULL	0	NULL	membrane potential 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin secretion from the pancreatic - cell is controlled by changes in membrane potential and intracellular Ca ( 2 + ) .
	manualset3
102202	5	401368	13	NULL	NULL	0	NULL	intracellular Ca ( 2 + )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin secretion from the pancreatic - cell is controlled by changes in membrane potential and intracellular Ca ( 2 + ) .
	manualset3
102203	1	401369	13	NULL	NULL	0	NULL	Insulin secretion 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin secretion was 50-60 % inhibited although islet glucose metabolism was unaffected and stimulus-induced ( Ca ( 2 + ) ) ( i ) rise was not ( 2 h ) or only marginally ( 5 h ) decreased .
	manualset3
102204	2	401369	13	NULL	NULL	0	NULL	50-60 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin secretion was 50-60 % inhibited although islet glucose metabolism was unaffected and stimulus-induced ( Ca ( 2 + ) ) ( i ) rise was not ( 2 h ) or only marginally ( 5 h ) decreased .
	manualset3
102205	3	401369	13	NULL	NULL	0	NULL	islet glucose metabolism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin secretion was 50-60 % inhibited although islet glucose metabolism was unaffected and stimulus-induced ( Ca ( 2 + ) ) ( i ) rise was not ( 2 h ) or only marginally ( 5 h ) decreased .
	manualset3
102206	4	401369	13	NULL	NULL	0	NULL	stimulus-induced ( Ca ( 2 + ) ) ( i ) rise	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin secretion was 50-60 % inhibited although islet glucose metabolism was unaffected and stimulus-induced ( Ca ( 2 + ) ) ( i ) rise was not ( 2 h ) or only marginally ( 5 h ) decreased .
	manualset3
102207	5	401369	13	NULL	NULL	0	NULL	2 h 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin secretion was 50-60 % inhibited although islet glucose metabolism was unaffected and stimulus-induced ( Ca ( 2 + ) ) ( i ) rise was not ( 2 h ) or only marginally ( 5 h ) decreased .
	manualset3
102208	6	401369	13	NULL	NULL	0	NULL	5 h 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin secretion was 50-60 % inhibited although islet glucose metabolism was unaffected and stimulus-induced ( Ca ( 2 + ) ) ( i ) rise was not ( 2 h ) or only marginally ( 5 h ) decreased .
	manualset3
102209	1	401370	13	NULL	NULL	0	NULL	Insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin stimulates glucose incorporation by 20-112 % into all the above pathways at glucose concentrations between 100 and 800 mg/dl .
	manualset3
102210	2	401370	13	NULL	NULL	0	NULL	glucose incorporation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin stimulates glucose incorporation by 20-112 % into all the above pathways at glucose concentrations between 100 and 800 mg/dl .
	manualset3
102211	3	401370	13	NULL	NULL	0	NULL	20-112 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin stimulates glucose incorporation by 20-112 % into all the above pathways at glucose concentrations between 100 and 800 mg/dl .
	manualset3
102212	4	401370	13	NULL	NULL	0	NULL	pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin stimulates glucose incorporation by 20-112 % into all the above pathways at glucose concentrations between 100 and 800 mg/dl .
	manualset3
102213	5	401370	13	NULL	NULL	0	NULL	glucose concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin stimulates glucose incorporation by 20-112 % into all the above pathways at glucose concentrations between 100 and 800 mg/dl .
	manualset3
102214	6	401370	13	NULL	NULL	0	NULL	between 100 and 800 mg/dl	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin stimulates glucose incorporation by 20-112 % into all the above pathways at glucose concentrations between 100 and 800 mg/dl .
	manualset3
102215	1	401371	13	NULL	NULL	0	NULL	Insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin was active in the physiological range ; 2 to 3 nM were sufficient to increase the induced delta-aminolevulinic acid synthetase to 50 % of the maximum effect obtained with a saturating amount of insulin ( 30 nM ) .
	manualset3
102216	2	401371	13	NULL	NULL	0	NULL	physiological range	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin was active in the physiological range ; 2 to 3 nM were sufficient to increase the induced delta-aminolevulinic acid synthetase to 50 % of the maximum effect obtained with a saturating amount of insulin ( 30 nM ) .
	manualset3
102217	3	401371	13	NULL	NULL	0	NULL	2 to 3 nM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin was active in the physiological range ; 2 to 3 nM were sufficient to increase the induced delta-aminolevulinic acid synthetase to 50 % of the maximum effect obtained with a saturating amount of insulin ( 30 nM ) .
	manualset3
102218	4	401371	13	NULL	NULL	0	NULL	delta-aminolevulinic acid synthetase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin was active in the physiological range ; 2 to 3 nM were sufficient to increase the induced delta-aminolevulinic acid synthetase to 50 % of the maximum effect obtained with a saturating amount of insulin ( 30 nM ) .
	manualset3
102219	5	401371	13	NULL	NULL	0	NULL	 50 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin was active in the physiological range ; 2 to 3 nM were sufficient to increase the induced delta-aminolevulinic acid synthetase to 50 % of the maximum effect obtained with a saturating amount of insulin ( 30 nM ) .
	manualset3
102220	6	401371	13	NULL	NULL	0	NULL	maximum effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin was active in the physiological range ; 2 to 3 nM were sufficient to increase the induced delta-aminolevulinic acid synthetase to 50 % of the maximum effect obtained with a saturating amount of insulin ( 30 nM ) .
	manualset3
102221	7	401371	13	NULL	NULL	0	NULL	amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin was active in the physiological range ; 2 to 3 nM were sufficient to increase the induced delta-aminolevulinic acid synthetase to 50 % of the maximum effect obtained with a saturating amount of insulin ( 30 nM ) .
	manualset3
102222	8	401371	13	NULL	NULL	0	NULL	insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin was active in the physiological range ; 2 to 3 nM were sufficient to increase the induced delta-aminolevulinic acid synthetase to 50 % of the maximum effect obtained with a saturating amount of insulin ( 30 nM ) .
	manualset3
102223	9	401371	13	NULL	NULL	0	NULL	30 nM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin was active in the physiological range ; 2 to 3 nM were sufficient to increase the induced delta-aminolevulinic acid synthetase to 50 % of the maximum effect obtained with a saturating amount of insulin ( 30 nM ) .
	manualset3
102224	1	401372	13	NULL	NULL	0	NULL	glucose responses 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrated incremental glucose , insulin and C-peptide responses were reduced by 47 % ( p & lt ; 0.001 ) , 23 % ( p & lt ; 0.05 ) and 15 % ( p & lt ; 0.05 ) , respectively .
	manualset3
102225	2	401372	13	NULL	NULL	0	NULL	insulin responses	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrated incremental glucose , insulin and C-peptide responses were reduced by 47 % ( p & lt ; 0.001 ) , 23 % ( p & lt ; 0.05 ) and 15 % ( p & lt ; 0.05 ) , respectively .
	manualset3
102226	3	401372	13	NULL	NULL	0	NULL	C-peptide responses	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrated incremental glucose , insulin and C-peptide responses were reduced by 47 % ( p & lt ; 0.001 ) , 23 % ( p & lt ; 0.05 ) and 15 % ( p & lt ; 0.05 ) , respectively .
	manualset3
102227	4	401372	13	NULL	NULL	0	NULL	47 % ( p & lt ; 0.001 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrated incremental glucose , insulin and C-peptide responses were reduced by 47 % ( p & lt ; 0.001 ) , 23 % ( p & lt ; 0.05 ) and 15 % ( p & lt ; 0.05 ) , respectively .
	manualset3
102228	5	401372	13	NULL	NULL	0	NULL	23 % ( p & lt ; 0.05 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrated incremental glucose , insulin and C-peptide responses were reduced by 47 % ( p & lt ; 0.001 ) , 23 % ( p & lt ; 0.05 ) and 15 % ( p & lt ; 0.05 ) , respectively .
	manualset3
102229	6	401372	13	NULL	NULL	0	NULL	15 % ( p & lt ; 0.05 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrated incremental glucose , insulin and C-peptide responses were reduced by 47 % ( p & lt ; 0.001 ) , 23 % ( p & lt ; 0.05 ) and 15 % ( p & lt ; 0.05 ) , respectively .
	manualset3
102230	1	401373	13	NULL	NULL	0	NULL	transcriptome analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrated transcriptome analysis of the cellular mechanisms associated with Ha-ras-dependent malignant transformation of the human breast epithelial MCF7 cell line .
	manualset3
102231	2	401373	13	NULL	NULL	0	NULL	 cellular mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrated transcriptome analysis of the cellular mechanisms associated with Ha-ras-dependent malignant transformation of the human breast epithelial MCF7 cell line .
	manualset3
102232	3	401373	13	NULL	NULL	0	NULL	Ha-ras-dependent malignant transformation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrated transcriptome analysis of the cellular mechanisms associated with Ha-ras-dependent malignant transformation of the human breast epithelial MCF7 cell line .
	manualset3
102233	4	401373	13	NULL	NULL	0	NULL	human breast epithelial MCF7 cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrated transcriptome analysis of the cellular mechanisms associated with Ha-ras-dependent malignant transformation of the human breast epithelial MCF7 cell line .
	manualset3
102234	1	401374	13	NULL	NULL	0	NULL	GIS	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrating GIS and fuzzy logic for urban solid waste management ( a case study of Sanandaj city , Iran ) .
	manualset3
102235	2	401374	13	NULL	NULL	0	NULL	fuzzy logic	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrating GIS and fuzzy logic for urban solid waste management ( a case study of Sanandaj city , Iran ) .
	manualset3
102236	3	401374	13	NULL	NULL	0	NULL	urban solid waste management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrating GIS and fuzzy logic for urban solid waste management ( a case study of Sanandaj city , Iran ) .
	manualset3
102237	4	401374	13	NULL	NULL	0	NULL	 case study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrating GIS and fuzzy logic for urban solid waste management ( a case study of Sanandaj city , Iran ) .
	manualset3
102238	5	401374	13	NULL	NULL	0	NULL	Sanandaj city	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrating GIS and fuzzy logic for urban solid waste management ( a case study of Sanandaj city , Iran ) .
	manualset3
102239	6	401374	13	NULL	NULL	0	NULL	Iran 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrating GIS and fuzzy logic for urban solid waste management ( a case study of Sanandaj city , Iran ) .
	manualset3
102240	1	401375	13	NULL	NULL	0	NULL	multiple program	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrating multiple program and policy approaches to hepatitis C prevention and care for injection drug users : a comprehensive approach .
	manualset3
102241	2	401375	13	NULL	NULL	NULL	NULL	policy approaches	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Integrating multiple program and policy approaches to hepatitis C prevention and care for injection drug users : a comprehensive approach .
	manualset3
102242	3	401375	13	NULL	NULL	0	NULL	 hepatitis C prevention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrating multiple program and policy approaches to hepatitis C prevention and care for injection drug users : a comprehensive approach .
	manualset3
102243	4	401375	13	NULL	NULL	0	NULL	care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrating multiple program and policy approaches to hepatitis C prevention and care for injection drug users : a comprehensive approach .
	manualset3
102244	5	401375	13	NULL	NULL	0	NULL	injection drug users 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrating multiple program and policy approaches to hepatitis C prevention and care for injection drug users : a comprehensive approach .
	manualset3
102245	6	401375	13	NULL	NULL	0	NULL	a comprehensive approach	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrating multiple program and policy approaches to hepatitis C prevention and care for injection drug users : a comprehensive approach .
	manualset3
102246	1	401376	13	NULL	NULL	0	NULL	Association study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Association study on the mitochondrial genome region np16181-16193 variation with type 2 diabetes mellitus ) .
	manualset3
102247	2	401376	13	NULL	NULL	0	NULL	mitochondrial genome region np16181-16193 variation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Association study on the mitochondrial genome region np16181-16193 variation with type 2 diabetes mellitus ) .
	manualset3
102248	3	401376	13	NULL	NULL	0	NULL	type 2 diabetes mellitus 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Association study on the mitochondrial genome region np16181-16193 variation with type 2 diabetes mellitus ) .
	manualset3
102249	1	401377	13	NULL	NULL	0	NULL	Integrative analyses 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrative analyses of genetic microsatellite data , cuticular hydrocarbons and behavioral assays showed that an individual acacia might be inhabited by the workers of several P. gracilis queens , whereas one P. ferrugineus colony monopolizes one or more host trees .
	manualset3
102250	2	401377	13	NULL	NULL	0	NULL	genetic microsatellite data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrative analyses of genetic microsatellite data , cuticular hydrocarbons and behavioral assays showed that an individual acacia might be inhabited by the workers of several P. gracilis queens , whereas one P. ferrugineus colony monopolizes one or more host trees .
	manualset3
102251	3	401377	13	NULL	NULL	0	NULL	cuticular hydrocarbons and behavioral assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrative analyses of genetic microsatellite data , cuticular hydrocarbons and behavioral assays showed that an individual acacia might be inhabited by the workers of several P. gracilis queens , whereas one P. ferrugineus colony monopolizes one or more host trees .
	manualset3
102252	4	401377	13	NULL	NULL	0	NULL	acacia	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrative analyses of genetic microsatellite data , cuticular hydrocarbons and behavioral assays showed that an individual acacia might be inhabited by the workers of several P. gracilis queens , whereas one P. ferrugineus colony monopolizes one or more host trees .
	manualset3
102253	5	401377	13	NULL	NULL	0	NULL	workers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrative analyses of genetic microsatellite data , cuticular hydrocarbons and behavioral assays showed that an individual acacia might be inhabited by the workers of several P. gracilis queens , whereas one P. ferrugineus colony monopolizes one or more host trees .
	manualset3
102254	6	401377	13	NULL	NULL	0	NULL	P. gracilis queens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrative analyses of genetic microsatellite data , cuticular hydrocarbons and behavioral assays showed that an individual acacia might be inhabited by the workers of several P. gracilis queens , whereas one P. ferrugineus colony monopolizes one or more host trees .
	manualset3
102255	7	401377	13	NULL	NULL	0	NULL	P. ferrugineus colony	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrative analyses of genetic microsatellite data , cuticular hydrocarbons and behavioral assays showed that an individual acacia might be inhabited by the workers of several P. gracilis queens , whereas one P. ferrugineus colony monopolizes one or more host trees .
	manualset3
102256	8	401377	13	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrative analyses of genetic microsatellite data , cuticular hydrocarbons and behavioral assays showed that an individual acacia might be inhabited by the workers of several P. gracilis queens , whereas one P. ferrugineus colony monopolizes one or more host trees .
	manualset3
102257	9	401377	13	NULL	NULL	0	NULL	host trees 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrative analyses of genetic microsatellite data , cuticular hydrocarbons and behavioral assays showed that an individual acacia might be inhabited by the workers of several P. gracilis queens , whereas one P. ferrugineus colony monopolizes one or more host trees .
	manualset3
102392	1	401378	13	NULL	NULL	0	NULL	Integrin-mediated type IV secretion 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrin-mediated type IV secretion by Helicobacter : what makes it tick ?
	manualset3
102393	2	401378	13	NULL	NULL	0	NULL	Helicobacter	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrin-mediated type IV secretion by Helicobacter : what makes it tick ?
	manualset3
102394	1	401379	13	NULL	NULL	0	NULL	Integrin 1/Akita double-knockout mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrin 1/Akita double-knockout mice on a Balb/c background develop advanced features of human diabetic nephropathy .
	manualset3
102395	2	401379	13	NULL	NULL	0	NULL	Balb/c background	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrin 1/Akita double-knockout mice on a Balb/c background develop advanced features of human diabetic nephropathy .
	manualset3
102396	3	401379	13	NULL	NULL	0	NULL	features	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrin 1/Akita double-knockout mice on a Balb/c background develop advanced features of human diabetic nephropathy .
	manualset3
102397	4	401379	13	NULL	NULL	0	NULL	human diabetic nephropathy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrin 1/Akita double-knockout mice on a Balb/c background develop advanced features of human diabetic nephropathy .
	manualset3
102398	1	401380	13	NULL	NULL	0	NULL	Integrins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrins as target : first phase III trial launches , but questions remain .
	manualset3
102399	2	401380	13	NULL	NULL	0	NULL	target	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrins as target : first phase III trial launches , but questions remain .
	manualset3
102400	3	401380	13	NULL	NULL	0	NULL	first phase III trial	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrins as target : first phase III trial launches , but questions remain .
	manualset3
102401	4	401380	13	NULL	NULL	0	NULL	questions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrins as target : first phase III trial launches , but questions remain .
	manualset3
102402	1	401381	13	NULL	NULL	0	NULL	Intense immunoreactivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intense immunoreactivity was noticed in several olfactory receptor neurons ( ORNs ) and their axonal fibers as they extend over the olfactory nerve , spread in the periphery of the olfactory bulb ( OB ) , and terminate in the glomerular layer .
	manualset3
102403	2	401381	13	NULL	NULL	0	NULL	several olfactory receptor neurons ( ORNs ) 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Intense immunoreactivity was noticed in several olfactory receptor neurons ( ORNs ) and their axonal fibers as they extend over the olfactory nerve , spread in the periphery of the olfactory bulb ( OB ) , and terminate in the glomerular layer .
	manualset3
102404	3	401381	13	NULL	NULL	0	NULL	axonal fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Intense immunoreactivity was noticed in several olfactory receptor neurons ( ORNs ) and their axonal fibers as they extend over the olfactory nerve , spread in the periphery of the olfactory bulb ( OB ) , and terminate in the glomerular layer .
	manualset3
102405	4	401381	13	NULL	NULL	0	NULL	olfactory nerve	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Intense immunoreactivity was noticed in several olfactory receptor neurons ( ORNs ) and their axonal fibers as they extend over the olfactory nerve , spread in the periphery of the olfactory bulb ( OB ) , and terminate in the glomerular layer .
	manualset3
102406	5	401381	13	NULL	NULL	0	NULL	periphery of the olfactory bulb ( OB )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Intense immunoreactivity was noticed in several olfactory receptor neurons ( ORNs ) and their axonal fibers as they extend over the olfactory nerve , spread in the periphery of the olfactory bulb ( OB ) , and terminate in the glomerular layer .
	manualset3
102407	6	401381	13	NULL	NULL	0	NULL	glomerular layer	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Intense immunoreactivity was noticed in several olfactory receptor neurons ( ORNs ) and their axonal fibers as they extend over the olfactory nerve , spread in the periphery of the olfactory bulb ( OB ) , and terminate in the glomerular layer .
	manualset3
102408	1	401382	13	NULL	NULL	0	NULL	Intensive care unit management 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intensive care unit management of liver transplant patients : a formidable challenge for the intensivist .
	manualset3
102409	2	401382	13	NULL	NULL	0	NULL	liver transplant patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Intensive care unit management of liver transplant patients : a formidable challenge for the intensivist .
	manualset3
102410	3	401382	13	NULL	NULL	0	NULL	formidable challenge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Intensive care unit management of liver transplant patients : a formidable challenge for the intensivist .
	manualset3
102411	4	401382	13	NULL	NULL	0	NULL	 intensivist	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Intensive care unit management of liver transplant patients : a formidable challenge for the intensivist .
	manualset3
102412	1	401383	13	NULL	NULL	0	NULL	Intensive care unit safety incidents	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intensive care unit safety incidents for medical versus surgical patients : a prospective multicenter study .
	manualset3
102413	2	401383	13	NULL	NULL	0	NULL	medical versus surgical patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Intensive care unit safety incidents for medical versus surgical patients : a prospective multicenter study .
	manualset3
102414	3	401383	13	NULL	NULL	0	NULL	prospective multicenter study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Intensive care unit safety incidents for medical versus surgical patients : a prospective multicenter study .
	manualset3
102415	1	401384	13	NULL	NULL	0	NULL	Intensive community pharmacy intervention 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intensive community pharmacy intervention had little impact on triptan consumption : a randomized controlled trial .
	manualset3
102416	2	401384	13	NULL	NULL	0	NULL	 impact 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intensive community pharmacy intervention had little impact on triptan consumption : a randomized controlled trial .
	manualset3
102417	3	401384	13	NULL	NULL	0	NULL	triptan	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Intensive community pharmacy intervention had little impact on triptan consumption : a randomized controlled trial .
	manualset3
102418	4	401384	13	NULL	NULL	0	NULL	consumption	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intensive community pharmacy intervention had little impact on triptan consumption : a randomized controlled trial .
	manualset3
102419	5	401384	13	NULL	NULL	0	NULL	trial 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Intensive community pharmacy intervention had little impact on triptan consumption : a randomized controlled trial .
	manualset3
102420	1	401385	13	NULL	NULL	0	NULL	Intensive glucose control 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intensive glucose control and cardiovascular outcomes .
	manualset3
102421	2	401385	13	NULL	NULL	0	NULL	cardiovascular outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intensive glucose control and cardiovascular outcomes .
	manualset3
102422	1	401386	13	NULL	NULL	0	NULL	Intensive training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Intensive training , IT tools are hallmarks of safety improvement program .
	manualset3
102423	2	401386	13	NULL	NULL	0	NULL	IT tools	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Intensive training , IT tools are hallmarks of safety improvement program .
	manualset3
102424	3	401386	13	NULL	NULL	0	NULL	hallmarks	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Intensive training , IT tools are hallmarks of safety improvement program .
	manualset3
102425	4	401386	13	NULL	NULL	0	NULL	safety improvement program	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Intensive training , IT tools are hallmarks of safety improvement program .
	manualset3
102426	1	401387	13	NULL	NULL	0	NULL	Inter-laboratory testing 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Inter - and intra-laboratory testing of the Daphnia magna IQ toxicity test .
	manualset3
102427	2	401387	13	NULL	NULL	0	NULL	intra-laboratory testing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Inter - and intra-laboratory testing of the Daphnia magna IQ toxicity test .
	manualset3
102428	3	401387	13	NULL	NULL	0	NULL	Daphnia magna IQ toxicity test 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Inter - and intra-laboratory testing of the Daphnia magna IQ toxicity test .
	manualset3
102429	1	401388	13	NULL	NULL	0	NULL	Interrater reliability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inter - and intrarater reliability of retrospective drug utilization reviewers .
	manualset3
102430	2	401388	13	NULL	NULL	0	NULL	intrarater reliability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inter - and intrarater reliability of retrospective drug utilization reviewers .
	manualset3
102431	3	401388	13	NULL	NULL	0	NULL	retrospective drug utilization 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inter - and intrarater reliability of retrospective drug utilization reviewers .
	manualset3
102432	4	401388	13	NULL	NULL	0	NULL	 reviewers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Inter - and intrarater reliability of retrospective drug utilization reviewers .
	manualset3
102433	1	401389	13	NULL	NULL	0	NULL	Interacting 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interacting with Congress : the President 's legislative liaison .
	manualset3
102434	2	401389	13	NULL	NULL	0	NULL	 Congress	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interacting with Congress : the President 's legislative liaison .
	manualset3
102435	3	401389	13	NULL	NULL	0	NULL	President 's	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Interacting with Congress : the President 's legislative liaison .
	manualset3
102436	4	401389	13	NULL	NULL	0	NULL	legislative liaison 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interacting with Congress : the President 's legislative liaison .
	manualset3
102437	1	401390	13	NULL	NULL	0	NULL	Interacting 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interacting with this receptor , PTHRP contributes to skeletal development through the regulation of chondrocyte proliferation and differentiation .
	manualset3
102438	2	401390	13	NULL	NULL	0	NULL	receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interacting with this receptor , PTHRP contributes to skeletal development through the regulation of chondrocyte proliferation and differentiation .
	manualset3
102439	3	401390	13	NULL	NULL	0	NULL	PTHRP 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interacting with this receptor , PTHRP contributes to skeletal development through the regulation of chondrocyte proliferation and differentiation .
	manualset3
102440	4	401390	13	NULL	NULL	0	NULL	skeletal development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interacting with this receptor , PTHRP contributes to skeletal development through the regulation of chondrocyte proliferation and differentiation .
	manualset3
102441	5	401390	13	NULL	NULL	0	NULL	regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interacting with this receptor , PTHRP contributes to skeletal development through the regulation of chondrocyte proliferation and differentiation .
	manualset3
102442	6	401390	13	NULL	NULL	0	NULL	chondrocyte proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interacting with this receptor , PTHRP contributes to skeletal development through the regulation of chondrocyte proliferation and differentiation .
	manualset3
102443	7	401390	13	NULL	NULL	0	NULL	chondrocyte differentiation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interacting with this receptor , PTHRP contributes to skeletal development through the regulation of chondrocyte proliferation and differentiation .
	manualset3
102444	1	401391	13	NULL	NULL	0	NULL	Interaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction between the platelet IIb/IIIa receptor gene and serotonin transporter gene is involved in the formation of the predisposition to myocardial infarction in young men .
	manualset3
102445	2	401391	13	NULL	NULL	0	NULL	platelet IIb/IIIa receptor gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction between the platelet IIb/IIIa receptor gene and serotonin transporter gene is involved in the formation of the predisposition to myocardial infarction in young men .
	manualset3
102446	3	401391	13	NULL	NULL	0	NULL	 serotonin transporter gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction between the platelet IIb/IIIa receptor gene and serotonin transporter gene is involved in the formation of the predisposition to myocardial infarction in young men .
	manualset3
102447	4	401391	13	NULL	NULL	0	NULL	formation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction between the platelet IIb/IIIa receptor gene and serotonin transporter gene is involved in the formation of the predisposition to myocardial infarction in young men .
	manualset3
102448	5	401391	13	NULL	NULL	0	NULL	predisposition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction between the platelet IIb/IIIa receptor gene and serotonin transporter gene is involved in the formation of the predisposition to myocardial infarction in young men .
	manualset3
102449	6	401391	13	NULL	NULL	0	NULL	myocardial infarction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction between the platelet IIb/IIIa receptor gene and serotonin transporter gene is involved in the formation of the predisposition to myocardial infarction in young men .
	manualset3
102450	7	401391	13	NULL	NULL	0	NULL	young men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction between the platelet IIb/IIIa receptor gene and serotonin transporter gene is involved in the formation of the predisposition to myocardial infarction in young men .
	manualset3
102451	1	401392	13	NULL	NULL	0	NULL	Interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of ASIC1 and ENaC subunits in human glioma cells and rat astrocytes .
	manualset3
102452	2	401392	13	NULL	NULL	0	NULL	ASIC1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of ASIC1 and ENaC subunits in human glioma cells and rat astrocytes .
	manualset3
102453	3	401392	13	NULL	NULL	0	NULL	ENaC subunits 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of ASIC1 and ENaC subunits in human glioma cells and rat astrocytes .
	manualset3
102454	4	401392	13	NULL	NULL	0	NULL	human glioma cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of ASIC1 and ENaC subunits in human glioma cells and rat astrocytes .
	manualset3
102455	5	401392	13	NULL	NULL	0	NULL	rat astrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of ASIC1 and ENaC subunits in human glioma cells and rat astrocytes .
	manualset3
102456	1	401393	13	NULL	NULL	0	NULL	Interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of activated Rab5 with actin-bundling proteins , L - and T-plastin and its relevance to endocytic functions in mammalian cells .
	manualset3
102457	2	401393	13	NULL	NULL	0	NULL	Rab5 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of activated Rab5 with actin-bundling proteins , L - and T-plastin and its relevance to endocytic functions in mammalian cells .
	manualset3
102458	3	401393	13	NULL	NULL	0	NULL	actin-bundling proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of activated Rab5 with actin-bundling proteins , L - and T-plastin and its relevance to endocytic functions in mammalian cells .
	manualset3
102459	4	401393	13	NULL	NULL	0	NULL	L -plastin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of activated Rab5 with actin-bundling proteins , L - and T-plastin and its relevance to endocytic functions in mammalian cells .
	manualset3
102460	5	401393	13	NULL	NULL	0	NULL	T-plastin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of activated Rab5 with actin-bundling proteins , L - and T-plastin and its relevance to endocytic functions in mammalian cells .
	manualset3
102461	6	401393	13	NULL	NULL	0	NULL	relevance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of activated Rab5 with actin-bundling proteins , L - and T-plastin and its relevance to endocytic functions in mammalian cells .
	manualset3
102462	7	401393	13	NULL	NULL	0	NULL	endocytic functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of activated Rab5 with actin-bundling proteins , L - and T-plastin and its relevance to endocytic functions in mammalian cells .
	manualset3
102463	8	401393	13	NULL	NULL	0	NULL	 mammalian cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of activated Rab5 with actin-bundling proteins , L - and T-plastin and its relevance to endocytic functions in mammalian cells .
	manualset3
102464	1	401394	13	NULL	NULL	0	NULL	308	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	308 patients enrolled and were randomized to three treatment groups : placebo , misoprostol 50 micrograms and misoprostol 200 micrograms .
	manualset3
102465	2	401394	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	308 patients enrolled and were randomized to three treatment groups : placebo , misoprostol 50 micrograms and misoprostol 200 micrograms .
	manualset3
102466	3	401394	13	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	308 patients enrolled and were randomized to three treatment groups : placebo , misoprostol 50 micrograms and misoprostol 200 micrograms .
	manualset3
102467	4	401394	13	NULL	NULL	0	NULL	treatment groups 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	308 patients enrolled and were randomized to three treatment groups : placebo , misoprostol 50 micrograms and misoprostol 200 micrograms .
	manualset3
102468	5	401394	13	NULL	NULL	0	NULL	 placebo	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	308 patients enrolled and were randomized to three treatment groups : placebo , misoprostol 50 micrograms and misoprostol 200 micrograms .
	manualset3
102469	6	401394	13	NULL	NULL	0	NULL	misoprostol 50 micrograms	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	308 patients enrolled and were randomized to three treatment groups : placebo , misoprostol 50 micrograms and misoprostol 200 micrograms .
	manualset3
102470	7	401394	13	NULL	NULL	0	NULL	misoprostol 200 micrograms 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	308 patients enrolled and were randomized to three treatment groups : placebo , misoprostol 50 micrograms and misoprostol 200 micrograms .
	manualset3
102471	1	401395	13	NULL	NULL	0	NULL	Interaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of adipokines and hepatitis B virus on histological liver injury in the Chinese .
	manualset3
102472	2	401395	13	NULL	NULL	0	NULL	adipokines 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of adipokines and hepatitis B virus on histological liver injury in the Chinese .
	manualset3
102473	3	401395	13	NULL	NULL	0	NULL	hepatitis B virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of adipokines and hepatitis B virus on histological liver injury in the Chinese .
	manualset3
102474	4	401395	13	NULL	NULL	0	NULL	histological liver injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of adipokines and hepatitis B virus on histological liver injury in the Chinese .
	manualset3
102475	5	401395	13	NULL	NULL	0	NULL	Chinese 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of adipokines and hepatitis B virus on histological liver injury in the Chinese .
	manualset3
102476	1	401396	13	NULL	NULL	0	NULL	Interaction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of date of eclosion with compositional changes of sugar and yeast but not with CR is responsible for life extension .
	manualset3
102477	2	401396	13	NULL	NULL	0	NULL	date	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of date of eclosion with compositional changes of sugar and yeast but not with CR is responsible for life extension .
	manualset3
102478	3	401396	13	NULL	NULL	0	NULL	eclosion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of date of eclosion with compositional changes of sugar and yeast but not with CR is responsible for life extension .
	manualset3
102479	4	401396	13	NULL	NULL	0	NULL	compositional changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of date of eclosion with compositional changes of sugar and yeast but not with CR is responsible for life extension .
	manualset3
102480	5	401396	13	NULL	NULL	0	NULL	sugar	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of date of eclosion with compositional changes of sugar and yeast but not with CR is responsible for life extension .
	manualset3
102481	6	401396	13	NULL	NULL	0	NULL	yeast 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of date of eclosion with compositional changes of sugar and yeast but not with CR is responsible for life extension .
	manualset3
102482	7	401396	13	NULL	NULL	0	NULL	CR	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of date of eclosion with compositional changes of sugar and yeast but not with CR is responsible for life extension .
	manualset3
102483	8	401396	13	NULL	NULL	0	NULL	life extension	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of date of eclosion with compositional changes of sugar and yeast but not with CR is responsible for life extension .
	manualset3
102484	1	401397	13	NULL	NULL	0	NULL	Interaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of methadone , reinforcement history , and variable-interval performance .
	manualset3
102485	2	401397	13	NULL	NULL	0	NULL	methadone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of methadone , reinforcement history , and variable-interval performance .
	manualset3
102486	3	401397	13	NULL	NULL	0	NULL	reinforcement history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of methadone , reinforcement history , and variable-interval performance .
	manualset3
102487	4	401397	13	NULL	NULL	0	NULL	variable-interval performance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of methadone , reinforcement history , and variable-interval performance .
	manualset3
102488	1	401398	13	NULL	NULL	0	NULL	Interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of somatostatin inhibition and dibutyryl cyclic AMP or potassium stimulation of growth hormone release from perifused rat pituitaries .
	manualset3
102489	2	401398	13	NULL	NULL	0	NULL	somatostatin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of somatostatin inhibition and dibutyryl cyclic AMP or potassium stimulation of growth hormone release from perifused rat pituitaries .
	manualset3
102490	3	401398	13	NULL	NULL	0	NULL	 inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of somatostatin inhibition and dibutyryl cyclic AMP or potassium stimulation of growth hormone release from perifused rat pituitaries .
	manualset3
102491	4	401398	13	NULL	NULL	0	NULL	dibutyryl cyclic AMP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of somatostatin inhibition and dibutyryl cyclic AMP or potassium stimulation of growth hormone release from perifused rat pituitaries .
	manualset3
102492	5	401398	13	NULL	NULL	0	NULL	potassium stimulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of somatostatin inhibition and dibutyryl cyclic AMP or potassium stimulation of growth hormone release from perifused rat pituitaries .
	manualset3
102493	6	401398	13	NULL	NULL	NULL	NULL	growth hormone release	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Interaction of somatostatin inhibition and dibutyryl cyclic AMP or potassium stimulation of growth hormone release from perifused rat pituitaries .
	manualset3
102494	7	401398	13	NULL	NULL	0	NULL	rat pituitaries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction of somatostatin inhibition and dibutyryl cyclic AMP or potassium stimulation of growth hormone release from perifused rat pituitaries .
	manualset3
102495	1	401399	13	NULL	NULL	0	NULL	Interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions between CD40 on APC and CD154 ( CD40L ) expressed by activated CD4 ( + ) T cells are crucially involved in formation and function of germinal centers ( GC ) , but mechanistic insight into these interactions remains limited .
	manualset3
102496	2	401399	13	NULL	NULL	0	NULL	 CD40 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions between CD40 on APC and CD154 ( CD40L ) expressed by activated CD4 ( + ) T cells are crucially involved in formation and function of germinal centers ( GC ) , but mechanistic insight into these interactions remains limited .
	manualset3
102497	3	401399	13	NULL	NULL	0	NULL	APC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions between CD40 on APC and CD154 ( CD40L ) expressed by activated CD4 ( + ) T cells are crucially involved in formation and function of germinal centers ( GC ) , but mechanistic insight into these interactions remains limited .
	manualset3
102498	4	401399	13	NULL	NULL	0	NULL	CD154 ( CD40L )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions between CD40 on APC and CD154 ( CD40L ) expressed by activated CD4 ( + ) T cells are crucially involved in formation and function of germinal centers ( GC ) , but mechanistic insight into these interactions remains limited .
	manualset3
102499	5	401399	13	NULL	NULL	0	NULL	CD4 ( + ) T cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions between CD40 on APC and CD154 ( CD40L ) expressed by activated CD4 ( + ) T cells are crucially involved in formation and function of germinal centers ( GC ) , but mechanistic insight into these interactions remains limited .
	manualset3
102500	6	401399	13	NULL	NULL	0	NULL	formation of germinal centers ( GC ) 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions between CD40 on APC and CD154 ( CD40L ) expressed by activated CD4 ( + ) T cells are crucially involved in formation and function of germinal centers ( GC ) , but mechanistic insight into these interactions remains limited .
	manualset3
102501	7	401399	13	NULL	NULL	0	NULL	function of germinal centers ( GC )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions between CD40 on APC and CD154 ( CD40L ) expressed by activated CD4 ( + ) T cells are crucially involved in formation and function of germinal centers ( GC ) , but mechanistic insight into these interactions remains limited .
	manualset3
102502	8	401399	13	NULL	NULL	0	NULL	mechanistic insight	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions between CD40 on APC and CD154 ( CD40L ) expressed by activated CD4 ( + ) T cells are crucially involved in formation and function of germinal centers ( GC ) , but mechanistic insight into these interactions remains limited .
	manualset3
102503	9	401399	13	NULL	NULL	0	NULL	interactions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions between CD40 on APC and CD154 ( CD40L ) expressed by activated CD4 ( + ) T cells are crucially involved in formation and function of germinal centers ( GC ) , but mechanistic insight into these interactions remains limited .
	manualset3
102504	1	401400	13	NULL	NULL	0	NULL	Interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions between angiotensin II and adrenoceptor-mediated effects on peripheral sympathetic neurotransmission were investigated in constant flow blood-perfused canine gracilis muscle in situ , without and with pretreatment by non-competitive alpha-adrenoceptor blockade .
	manualset3
102505	2	401400	13	NULL	NULL	0	NULL	angiotensin II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions between angiotensin II and adrenoceptor-mediated effects on peripheral sympathetic neurotransmission were investigated in constant flow blood-perfused canine gracilis muscle in situ , without and with pretreatment by non-competitive alpha-adrenoceptor blockade .
	manualset3
102506	3	401400	13	NULL	NULL	0	NULL	adrenoceptor-mediated effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions between angiotensin II and adrenoceptor-mediated effects on peripheral sympathetic neurotransmission were investigated in constant flow blood-perfused canine gracilis muscle in situ , without and with pretreatment by non-competitive alpha-adrenoceptor blockade .
	manualset3
102507	4	401400	13	NULL	NULL	0	NULL	peripheral sympathetic neurotransmission	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions between angiotensin II and adrenoceptor-mediated effects on peripheral sympathetic neurotransmission were investigated in constant flow blood-perfused canine gracilis muscle in situ , without and with pretreatment by non-competitive alpha-adrenoceptor blockade .
	manualset3
102508	5	401400	13	NULL	NULL	NULL	NULL	constant flow 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Interactions between angiotensin II and adrenoceptor-mediated effects on peripheral sympathetic neurotransmission were investigated in constant flow blood-perfused canine gracilis muscle in situ , without and with pretreatment by non-competitive alpha-adrenoceptor blockade .
	manualset3
102509	6	401400	13	NULL	NULL	0	NULL	canine gracilis muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions between angiotensin II and adrenoceptor-mediated effects on peripheral sympathetic neurotransmission were investigated in constant flow blood-perfused canine gracilis muscle in situ , without and with pretreatment by non-competitive alpha-adrenoceptor blockade .
	manualset3
102510	7	401400	13	NULL	NULL	NULL	NULL	 pretreatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Interactions between angiotensin II and adrenoceptor-mediated effects on peripheral sympathetic neurotransmission were investigated in constant flow blood-perfused canine gracilis muscle in situ , without and with pretreatment by non-competitive alpha-adrenoceptor blockade .
	manualset3
102511	8	401400	13	NULL	NULL	0	NULL	 alpha-adrenoceptor blockade 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions between angiotensin II and adrenoceptor-mediated effects on peripheral sympathetic neurotransmission were investigated in constant flow blood-perfused canine gracilis muscle in situ , without and with pretreatment by non-competitive alpha-adrenoceptor blockade .
	manualset3
102512	1	401401	13	NULL	NULL	0	NULL	Interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions between the collagen fibrils and other extracellular matrix molecules maintain structural integrity of cartilage , orchestrate complex dynamic events during embryonic development , and help to regulate fibrillogenesis .
	manualset3
102513	2	401401	13	NULL	NULL	0	NULL	collagen fibrils	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions between the collagen fibrils and other extracellular matrix molecules maintain structural integrity of cartilage , orchestrate complex dynamic events during embryonic development , and help to regulate fibrillogenesis .
	manualset3
102514	3	401401	13	NULL	NULL	0	NULL	extracellular matrix molecules 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions between the collagen fibrils and other extracellular matrix molecules maintain structural integrity of cartilage , orchestrate complex dynamic events during embryonic development , and help to regulate fibrillogenesis .
	manualset3
102515	4	401401	13	NULL	NULL	0	NULL	structural integrity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions between the collagen fibrils and other extracellular matrix molecules maintain structural integrity of cartilage , orchestrate complex dynamic events during embryonic development , and help to regulate fibrillogenesis .
	manualset3
102516	5	401401	13	NULL	NULL	0	NULL	cartilage	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions between the collagen fibrils and other extracellular matrix molecules maintain structural integrity of cartilage , orchestrate complex dynamic events during embryonic development , and help to regulate fibrillogenesis .
	manualset3
102517	6	401401	13	NULL	NULL	0	NULL	dynamic events	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions between the collagen fibrils and other extracellular matrix molecules maintain structural integrity of cartilage , orchestrate complex dynamic events during embryonic development , and help to regulate fibrillogenesis .
	manualset3
102518	7	401401	13	NULL	NULL	0	NULL	embryonic development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions between the collagen fibrils and other extracellular matrix molecules maintain structural integrity of cartilage , orchestrate complex dynamic events during embryonic development , and help to regulate fibrillogenesis .
	manualset3
102519	8	401401	13	NULL	NULL	0	NULL	fibrillogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions between the collagen fibrils and other extracellular matrix molecules maintain structural integrity of cartilage , orchestrate complex dynamic events during embryonic development , and help to regulate fibrillogenesis .
	manualset3
102521	1	401402	13	NULL	NULL	0	NULL	Interactions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions of hematopoietic cells with their microenvironment control blood cell colonization , homing and hematopoiesis .
	manualset3
102522	2	401402	13	NULL	NULL	0	NULL	hematopoietic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions of hematopoietic cells with their microenvironment control blood cell colonization , homing and hematopoiesis .
	manualset3
102523	3	401402	13	NULL	NULL	0	NULL	microenvironment	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions of hematopoietic cells with their microenvironment control blood cell colonization , homing and hematopoiesis .
	manualset3
102524	4	401402	13	NULL	NULL	0	NULL	 blood cell colonization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions of hematopoietic cells with their microenvironment control blood cell colonization , homing and hematopoiesis .
	manualset3
102525	5	401402	13	NULL	NULL	0	NULL	homing 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions of hematopoietic cells with their microenvironment control blood cell colonization , homing and hematopoiesis .
	manualset3
102526	6	401402	13	NULL	NULL	0	NULL	hematopoiesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions of hematopoietic cells with their microenvironment control blood cell colonization , homing and hematopoiesis .
	manualset3
102527	1	401403	13	NULL	NULL	0	NULL	Interactions 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions of magnetic-fluid-loaded liposomes ( MFL ) with human adenocarcinoma prostatic cell line PC3 were investigated in vitro .
	manualset3
102528	2	401403	13	NULL	NULL	0	NULL	magnetic-fluid-loaded liposomes ( MFL )	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions of magnetic-fluid-loaded liposomes ( MFL ) with human adenocarcinoma prostatic cell line PC3 were investigated in vitro .
	manualset3
102529	3	401403	13	NULL	NULL	0	NULL	human adenocarcinoma prostatic cell line PC3 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions of magnetic-fluid-loaded liposomes ( MFL ) with human adenocarcinoma prostatic cell line PC3 were investigated in vitro .
	manualset3
102530	1	401404	13	NULL	NULL	0	NULL	Interactive effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactive effects of thermal environment and energy intake on thyroid hormone metabolism in newborn pigs .
	manualset3
102531	2	401404	13	NULL	NULL	0	NULL	thermal environment 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactive effects of thermal environment and energy intake on thyroid hormone metabolism in newborn pigs .
	manualset3
102532	3	401404	13	NULL	NULL	0	NULL	energy intake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactive effects of thermal environment and energy intake on thyroid hormone metabolism in newborn pigs .
	manualset3
102533	4	401404	13	NULL	NULL	0	NULL	thyroid hormone metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactive effects of thermal environment and energy intake on thyroid hormone metabolism in newborn pigs .
	manualset3
102534	5	401404	13	NULL	NULL	0	NULL	newborn pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactive effects of thermal environment and energy intake on thyroid hormone metabolism in newborn pigs .
	manualset3
102535	1	401405	13	NULL	NULL	0	NULL	Interbehavioral psychology 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Interbehavioral psychology and radical behaviorism : Some similarities and differences .
	manualset3
102536	2	401405	13	NULL	NULL	0	NULL	radical behaviorism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Interbehavioral psychology and radical behaviorism : Some similarities and differences .
	manualset3
102537	3	401405	13	NULL	NULL	0	NULL	similarities	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Interbehavioral psychology and radical behaviorism : Some similarities and differences .
	manualset3
102538	4	401405	13	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Interbehavioral psychology and radical behaviorism : Some similarities and differences .
	manualset3
102539	1	401406	13	NULL	NULL	0	NULL	Intercell mediators	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Intercell mediators , or cytokines , are released on tissue stimulation or as a result of mild damage .
	manualset3
102540	2	401406	13	NULL	NULL	0	NULL	cytokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Intercell mediators , or cytokines , are released on tissue stimulation or as a result of mild damage .
	manualset3
102541	3	401406	13	NULL	NULL	0	NULL	tissue stimulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intercell mediators , or cytokines , are released on tissue stimulation or as a result of mild damage .
	manualset3
102542	4	401406	13	NULL	NULL	NULL	NULL	result	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Intercell mediators , or cytokines , are released on tissue stimulation or as a result of mild damage .
	manualset3
102543	5	401406	13	NULL	NULL	0	NULL	mild damage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intercell mediators , or cytokines , are released on tissue stimulation or as a result of mild damage .
	manualset3
102544	1	401407	13	NULL	NULL	0	NULL	Intercellular aggregation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intercellular aggregation in this system is mediated by the binding of the Fc portions of IgG antibodies on the spleen cells with Fc receptors ( Fc gamma R ) on P388D1 .
	manualset3
102545	2	401407	13	NULL	NULL	0	NULL	system	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Intercellular aggregation in this system is mediated by the binding of the Fc portions of IgG antibodies on the spleen cells with Fc receptors ( Fc gamma R ) on P388D1 .
	manualset3
102546	3	401407	13	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intercellular aggregation in this system is mediated by the binding of the Fc portions of IgG antibodies on the spleen cells with Fc receptors ( Fc gamma R ) on P388D1 .
	manualset3
102547	4	401407	13	NULL	NULL	0	NULL	Fc portions of IgG antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Intercellular aggregation in this system is mediated by the binding of the Fc portions of IgG antibodies on the spleen cells with Fc receptors ( Fc gamma R ) on P388D1 .
	manualset3
102548	5	401407	13	NULL	NULL	0	NULL	spleen cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Intercellular aggregation in this system is mediated by the binding of the Fc portions of IgG antibodies on the spleen cells with Fc receptors ( Fc gamma R ) on P388D1 .
	manualset3
102549	6	401407	13	NULL	NULL	0	NULL	Fc receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Intercellular aggregation in this system is mediated by the binding of the Fc portions of IgG antibodies on the spleen cells with Fc receptors ( Fc gamma R ) on P388D1 .
	manualset3
102550	7	401407	13	NULL	NULL	0	NULL	 Fc gamma R	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Intercellular aggregation in this system is mediated by the binding of the Fc portions of IgG antibodies on the spleen cells with Fc receptors ( Fc gamma R ) on P388D1 .
	manualset3
102551	8	401407	13	NULL	NULL	0	NULL	P388D1	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Intercellular aggregation in this system is mediated by the binding of the Fc portions of IgG antibodies on the spleen cells with Fc receptors ( Fc gamma R ) on P388D1 .
	manualset3
102552	1	401408	13	NULL	NULL	0	NULL	Intercrosses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intercrosses of IRS-2 ( + / - ) IRS-3 ( + / - ) mice yielded nine genotypes , and all of them including IRS-2 ( - / - ) IRS-3 ( - / - ) mice were apparently healthy and showed normal growth .
	manualset3
102553	2	401408	13	NULL	NULL	NULL	NULL	IRS-2 ( + / - ) IRS-3 ( + / - ) mice 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Intercrosses of IRS-2 ( + / - ) IRS-3 ( + / - ) mice yielded nine genotypes , and all of them including IRS-2 ( - / - ) IRS-3 ( - / - ) mice were apparently healthy and showed normal growth .
	manualset3
102554	3	401408	13	NULL	NULL	NULL	NULL	nine genotypes	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Intercrosses of IRS-2 ( + / - ) IRS-3 ( + / - ) mice yielded nine genotypes , and all of them including IRS-2 ( - / - ) IRS-3 ( - / - ) mice were apparently healthy and showed normal growth .
	manualset3
102555	4	401408	13	NULL	NULL	0	NULL	IRS-2 ( - / - ) IRS-3 ( - / - ) mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Intercrosses of IRS-2 ( + / - ) IRS-3 ( + / - ) mice yielded nine genotypes , and all of them including IRS-2 ( - / - ) IRS-3 ( - / - ) mice were apparently healthy and showed normal growth .
	manualset3
102556	5	401408	13	NULL	NULL	0	NULL	normal growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intercrosses of IRS-2 ( + / - ) IRS-3 ( + / - ) mice yielded nine genotypes , and all of them including IRS-2 ( - / - ) IRS-3 ( - / - ) mice were apparently healthy and showed normal growth .
	manualset3
102557	1	401409	13	NULL	NULL	0	NULL	Interdisciplinary research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Interdisciplinary research : a philosophy , art form , artifact or antidote ?
	manualset3
102558	2	401409	13	NULL	NULL	0	NULL	philosophy	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Interdisciplinary research : a philosophy , art form , artifact or antidote ?
	manualset3
102559	3	401409	13	NULL	NULL	0	NULL	art form	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Interdisciplinary research : a philosophy , art form , artifact or antidote ?
	manualset3
102560	4	401409	13	NULL	NULL	0	NULL	artifact	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Interdisciplinary research : a philosophy , art form , artifact or antidote ?
	manualset3
102561	5	401409	13	NULL	NULL	0	NULL	antidote 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Interdisciplinary research : a philosophy , art form , artifact or antidote ?
	manualset3
102562	1	401410	13	NULL	NULL	0	NULL	16.2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , 16.2 % of patients were positive for both thyroid and pancreatic antibodies .
	manualset3
102563	2	401410	13	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , 16.2 % of patients were positive for both thyroid and pancreatic antibodies .
	manualset3
102564	3	401410	13	NULL	NULL	0	NULL	thyroid antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , 16.2 % of patients were positive for both thyroid and pancreatic antibodies .
	manualset3
102565	4	401410	13	NULL	NULL	0	NULL	 pancreatic antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , 16.2 % of patients were positive for both thyroid and pancreatic antibodies .
	manualset3
102566	1	401411	13	NULL	NULL	0	NULL	21 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , 21 % of them , mostly involved in membrane transport and protein metabolism , showed a n-hexadecane-dependent regulation with regulatory proteins such as CRP likely to have a key role in M145-AH n-hexadecane growth .
	manualset3
102567	2	401411	13	NULL	NULL	0	NULL	membrane transport	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , 21 % of them , mostly involved in membrane transport and protein metabolism , showed a n-hexadecane-dependent regulation with regulatory proteins such as CRP likely to have a key role in M145-AH n-hexadecane growth .
	manualset3
102568	3	401411	13	NULL	NULL	0	NULL	protein metabolism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , 21 % of them , mostly involved in membrane transport and protein metabolism , showed a n-hexadecane-dependent regulation with regulatory proteins such as CRP likely to have a key role in M145-AH n-hexadecane growth .
	manualset3
102569	4	401411	13	NULL	NULL	0	NULL	n-hexadecane-dependent regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , 21 % of them , mostly involved in membrane transport and protein metabolism , showed a n-hexadecane-dependent regulation with regulatory proteins such as CRP likely to have a key role in M145-AH n-hexadecane growth .
	manualset3
102570	5	401411	13	NULL	NULL	0	NULL	regulatory proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , 21 % of them , mostly involved in membrane transport and protein metabolism , showed a n-hexadecane-dependent regulation with regulatory proteins such as CRP likely to have a key role in M145-AH n-hexadecane growth .
	manualset3
102571	6	401411	13	NULL	NULL	0	NULL	 CRP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , 21 % of them , mostly involved in membrane transport and protein metabolism , showed a n-hexadecane-dependent regulation with regulatory proteins such as CRP likely to have a key role in M145-AH n-hexadecane growth .
	manualset3
102572	7	401411	13	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , 21 % of them , mostly involved in membrane transport and protein metabolism , showed a n-hexadecane-dependent regulation with regulatory proteins such as CRP likely to have a key role in M145-AH n-hexadecane growth .
	manualset3
102573	8	401411	13	NULL	NULL	0	NULL	M145-AH n-hexadecane growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , 21 % of them , mostly involved in membrane transport and protein metabolism , showed a n-hexadecane-dependent regulation with regulatory proteins such as CRP likely to have a key role in M145-AH n-hexadecane growth .
	manualset3
102574	1	401412	13	NULL	NULL	0	NULL	Gsp1p	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , Gsp1p was found to interact genetically and physically with the telomeric component Sir4p .
	manualset3
102575	2	401412	13	NULL	NULL	0	NULL	telomeric component 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , Gsp1p was found to interact genetically and physically with the telomeric component Sir4p .
	manualset3
102576	3	401412	13	NULL	NULL	0	NULL	Sir4p	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , Gsp1p was found to interact genetically and physically with the telomeric component Sir4p .
	manualset3
102577	1	401413	13	NULL	NULL	0	NULL	31P NMR spectra	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	31P NMR spectra indicate the occurrence of a similar complexation in RBC cryolysates .
	manualset3
102578	2	401413	13	NULL	NULL	0	NULL	occurrence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	31P NMR spectra indicate the occurrence of a similar complexation in RBC cryolysates .
	manualset3
102579	3	401413	13	NULL	NULL	0	NULL	complexation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	31P NMR spectra indicate the occurrence of a similar complexation in RBC cryolysates .
	manualset3
102580	4	401413	13	NULL	NULL	0	NULL	RBC cryolysates	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	31P NMR spectra indicate the occurrence of a similar complexation in RBC cryolysates .
	manualset3
102581	1	401414	13	NULL	NULL	0	NULL	RIP-HGF transgenic mouse beta-cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , RIP-HGF transgenic mouse beta-cells and normal beta-cells treated with HGF display increased sensitivity to palmitate-mediated apoptosis in vitro .
	manualset3
102582	2	401414	13	NULL	NULL	0	NULL	normal beta-cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , RIP-HGF transgenic mouse beta-cells and normal beta-cells treated with HGF display increased sensitivity to palmitate-mediated apoptosis in vitro .
	manualset3
102583	3	401414	13	NULL	NULL	0	NULL	HGF 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , RIP-HGF transgenic mouse beta-cells and normal beta-cells treated with HGF display increased sensitivity to palmitate-mediated apoptosis in vitro .
	manualset3
102585	5	401414	13	NULL	NULL	0	NULL	sensitivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , RIP-HGF transgenic mouse beta-cells and normal beta-cells treated with HGF display increased sensitivity to palmitate-mediated apoptosis in vitro .
	manualset3
102586	6	401414	13	NULL	NULL	0	NULL	palmitate-mediated apoptosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , RIP-HGF transgenic mouse beta-cells and normal beta-cells treated with HGF display increased sensitivity to palmitate-mediated apoptosis in vitro .
	manualset3
102587	1	401415	13	NULL	NULL	0	NULL	Rab3 binding proteins ( RIMs )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , Rab3 binding proteins ( RIMs ) , a diverse multidomain family of proteins that operate as effectors of the small G protein Rab3 involved in secretory vesicle trafficking , have recently identified as binding partners of Ca ( V ) channels , placing both proteins in the center of an interaction network in the molecular anatomy of the active zones that influence different aspects of secretion .
	manualset3
102588	2	401415	13	NULL	NULL	0	NULL	a diverse multidomain family of proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , Rab3 binding proteins ( RIMs ) , a diverse multidomain family of proteins that operate as effectors of the small G protein Rab3 involved in secretory vesicle trafficking , have recently identified as binding partners of Ca ( V ) channels , placing both proteins in the center of an interaction network in the molecular anatomy of the active zones that influence different aspects of secretion .
	manualset3
102589	3	401415	13	NULL	NULL	NULL	NULL	effectors	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Interestingly , Rab3 binding proteins ( RIMs ) , a diverse multidomain family of proteins that operate as effectors of the small G protein Rab3 involved in secretory vesicle trafficking , have recently identified as binding partners of Ca ( V ) channels , placing both proteins in the center of an interaction network in the molecular anatomy of the active zones that influence different aspects of secretion .
	manualset3
102590	4	401415	13	NULL	NULL	0	NULL	small G protein Rab3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , Rab3 binding proteins ( RIMs ) , a diverse multidomain family of proteins that operate as effectors of the small G protein Rab3 involved in secretory vesicle trafficking , have recently identified as binding partners of Ca ( V ) channels , placing both proteins in the center of an interaction network in the molecular anatomy of the active zones that influence different aspects of secretion .
	manualset3
102591	5	401415	13	NULL	NULL	NULL	NULL	 secretory vesicle trafficking	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Interestingly , Rab3 binding proteins ( RIMs ) , a diverse multidomain family of proteins that operate as effectors of the small G protein Rab3 involved in secretory vesicle trafficking , have recently identified as binding partners of Ca ( V ) channels , placing both proteins in the center of an interaction network in the molecular anatomy of the active zones that influence different aspects of secretion .
	manualset3
102592	6	401415	13	NULL	NULL	0	NULL	binding partners of Ca ( V ) channels	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , Rab3 binding proteins ( RIMs ) , a diverse multidomain family of proteins that operate as effectors of the small G protein Rab3 involved in secretory vesicle trafficking , have recently identified as binding partners of Ca ( V ) channels , placing both proteins in the center of an interaction network in the molecular anatomy of the active zones that influence different aspects of secretion .
	manualset3
102593	7	401415	13	NULL	NULL	0	NULL	proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , Rab3 binding proteins ( RIMs ) , a diverse multidomain family of proteins that operate as effectors of the small G protein Rab3 involved in secretory vesicle trafficking , have recently identified as binding partners of Ca ( V ) channels , placing both proteins in the center of an interaction network in the molecular anatomy of the active zones that influence different aspects of secretion .
	manualset3
102594	8	401415	13	NULL	NULL	0	NULL	center of an interaction network	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , Rab3 binding proteins ( RIMs ) , a diverse multidomain family of proteins that operate as effectors of the small G protein Rab3 involved in secretory vesicle trafficking , have recently identified as binding partners of Ca ( V ) channels , placing both proteins in the center of an interaction network in the molecular anatomy of the active zones that influence different aspects of secretion .
	manualset3
102595	9	401415	13	NULL	NULL	0	NULL	molecular anatomy 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , Rab3 binding proteins ( RIMs ) , a diverse multidomain family of proteins that operate as effectors of the small G protein Rab3 involved in secretory vesicle trafficking , have recently identified as binding partners of Ca ( V ) channels , placing both proteins in the center of an interaction network in the molecular anatomy of the active zones that influence different aspects of secretion .
	manualset3
102596	10	401415	13	NULL	NULL	0	NULL	active zones	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , Rab3 binding proteins ( RIMs ) , a diverse multidomain family of proteins that operate as effectors of the small G protein Rab3 involved in secretory vesicle trafficking , have recently identified as binding partners of Ca ( V ) channels , placing both proteins in the center of an interaction network in the molecular anatomy of the active zones that influence different aspects of secretion .
	manualset3
102597	11	401415	13	NULL	NULL	0	NULL	 influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , Rab3 binding proteins ( RIMs ) , a diverse multidomain family of proteins that operate as effectors of the small G protein Rab3 involved in secretory vesicle trafficking , have recently identified as binding partners of Ca ( V ) channels , placing both proteins in the center of an interaction network in the molecular anatomy of the active zones that influence different aspects of secretion .
	manualset3
102598	12	401415	13	NULL	NULL	0	NULL	different aspects of secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , Rab3 binding proteins ( RIMs ) , a diverse multidomain family of proteins that operate as effectors of the small G protein Rab3 involved in secretory vesicle trafficking , have recently identified as binding partners of Ca ( V ) channels , placing both proteins in the center of an interaction network in the molecular anatomy of the active zones that influence different aspects of secretion .
	manualset3
102599	1	401416	13	NULL	NULL	0	NULL	 reciprocal relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , a reciprocal relationship was observed between femoral geometry and material stiffness ; this relationship may have contributed to the brittle phenotype of A/J femurs .
	manualset3
102600	2	401416	13	NULL	NULL	0	NULL	femoral geometry	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , a reciprocal relationship was observed between femoral geometry and material stiffness ; this relationship may have contributed to the brittle phenotype of A/J femurs .
	manualset3
102601	3	401416	13	NULL	NULL	0	NULL	material stiffness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , a reciprocal relationship was observed between femoral geometry and material stiffness ; this relationship may have contributed to the brittle phenotype of A/J femurs .
	manualset3
102602	4	401416	13	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , a reciprocal relationship was observed between femoral geometry and material stiffness ; this relationship may have contributed to the brittle phenotype of A/J femurs .
	manualset3
102603	5	401416	13	NULL	NULL	0	NULL	brittle phenotype of A/J femurs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , a reciprocal relationship was observed between femoral geometry and material stiffness ; this relationship may have contributed to the brittle phenotype of A/J femurs .
	manualset3
102604	1	401417	13	NULL	NULL	0	NULL	cytokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , both cytokines act principally on keratinocytes and do not impact the immune system .
	manualset3
102605	2	401417	13	NULL	NULL	0	NULL	keratinocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , both cytokines act principally on keratinocytes and do not impact the immune system .
	manualset3
102607	4	401417	13	NULL	NULL	0	NULL	immune system	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , both cytokines act principally on keratinocytes and do not impact the immune system .
	manualset3
102608	1	401418	13	NULL	NULL	0	NULL	five compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , five compounds show a rather good - secretase inhibitory potency while they retain their ability to inhibit AChE and/or BuChE activity .
	manualset3
102609	2	401418	13	NULL	NULL	0	NULL	secretase inhibitory potency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , five compounds show a rather good - secretase inhibitory potency while they retain their ability to inhibit AChE and/or BuChE activity .
	manualset3
102610	3	401418	13	NULL	NULL	0	NULL	ability 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , five compounds show a rather good - secretase inhibitory potency while they retain their ability to inhibit AChE and/or BuChE activity .
	manualset3
102611	4	401418	13	NULL	NULL	0	NULL	AChE activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , five compounds show a rather good - secretase inhibitory potency while they retain their ability to inhibit AChE and/or BuChE activity .
	manualset3
102612	5	401418	13	NULL	NULL	0	NULL	BuChE activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , five compounds show a rather good - secretase inhibitory potency while they retain their ability to inhibit AChE and/or BuChE activity .
	manualset3
102613	1	401419	13	NULL	NULL	0	NULL	Adriamycin treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , following Adriamycin treatment , the levels of Fas decreased in the wild-type mice .
	manualset3
102614	2	401419	13	NULL	NULL	0	NULL	levels of Fas 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , following Adriamycin treatment , the levels of Fas decreased in the wild-type mice .
	manualset3
102615	3	401419	13	NULL	NULL	0	NULL	wild-type mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , following Adriamycin treatment , the levels of Fas decreased in the wild-type mice .
	manualset3
102616	1	401420	13	NULL	NULL	NULL	NULL	overexpression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Interestingly , forced overexpression of Aurora B increased the protein levels of survivin , but not those of a non-phosphorylatable survivin mutant in which threonine 117 was replaced by alanine , indicating that phosphorylation of survivin is required for this effect .
	manualset3
102617	3	401420	13	NULL	NULL	NULL	NULL	protein levels 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Interestingly , forced overexpression of Aurora B increased the protein levels of survivin , but not those of a non-phosphorylatable survivin mutant in which threonine 117 was replaced by alanine , indicating that phosphorylation of survivin is required for this effect .
	manualset3
102618	3	401420	13	NULL	NULL	0	NULL	survivin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , forced overexpression of Aurora B increased the protein levels of survivin , but not those of a non-phosphorylatable survivin mutant in which threonine 117 was replaced by alanine , indicating that phosphorylation of survivin is required for this effect .
	manualset3
102619	4	401420	13	NULL	NULL	0	NULL	non-phosphorylatable survivin mutant 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , forced overexpression of Aurora B increased the protein levels of survivin , but not those of a non-phosphorylatable survivin mutant in which threonine 117 was replaced by alanine , indicating that phosphorylation of survivin is required for this effect .
	manualset3
102620	5	401420	13	NULL	NULL	0	NULL	threonine 117	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , forced overexpression of Aurora B increased the protein levels of survivin , but not those of a non-phosphorylatable survivin mutant in which threonine 117 was replaced by alanine , indicating that phosphorylation of survivin is required for this effect .
	manualset3
102621	6	401420	13	NULL	NULL	0	NULL	alanine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , forced overexpression of Aurora B increased the protein levels of survivin , but not those of a non-phosphorylatable survivin mutant in which threonine 117 was replaced by alanine , indicating that phosphorylation of survivin is required for this effect .
	manualset3
102622	7	401420	13	NULL	NULL	0	NULL	phosphorylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , forced overexpression of Aurora B increased the protein levels of survivin , but not those of a non-phosphorylatable survivin mutant in which threonine 117 was replaced by alanine , indicating that phosphorylation of survivin is required for this effect .
	manualset3
102623	8	401420	13	NULL	NULL	0	NULL	survivin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , forced overexpression of Aurora B increased the protein levels of survivin , but not those of a non-phosphorylatable survivin mutant in which threonine 117 was replaced by alanine , indicating that phosphorylation of survivin is required for this effect .
	manualset3
102624	9	401420	13	NULL	NULL	0	NULL	effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , forced overexpression of Aurora B increased the protein levels of survivin , but not those of a non-phosphorylatable survivin mutant in which threonine 117 was replaced by alanine , indicating that phosphorylation of survivin is required for this effect .
	manualset3
102625	2	401420	13	NULL	NULL	0	NULL	Aurora B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , forced overexpression of Aurora B increased the protein levels of survivin , but not those of a non-phosphorylatable survivin mutant in which threonine 117 was replaced by alanine , indicating that phosphorylation of survivin is required for this effect .
	manualset3
102626	1	401421	13	NULL	NULL	0	NULL	immune cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , immune cells do not appear to express specific IL-24 receptor chains ( IL-20R1 / IL-20R2 and IL-22R / IL-20R2 ) , it is therefore unlikely that IL-24 has classical immune-modulating properties .
	manualset3
102627	2	401421	13	NULL	NULL	0	NULL	IL-24 receptor chains	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , immune cells do not appear to express specific IL-24 receptor chains ( IL-20R1 / IL-20R2 and IL-22R / IL-20R2 ) , it is therefore unlikely that IL-24 has classical immune-modulating properties .
	manualset3
102628	3	401421	13	NULL	NULL	0	NULL	 IL-20R1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , immune cells do not appear to express specific IL-24 receptor chains ( IL-20R1 / IL-20R2 and IL-22R / IL-20R2 ) , it is therefore unlikely that IL-24 has classical immune-modulating properties .
	manualset3
102629	4	401421	13	NULL	NULL	0	NULL	IL-20R2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , immune cells do not appear to express specific IL-24 receptor chains ( IL-20R1 / IL-20R2 and IL-22R / IL-20R2 ) , it is therefore unlikely that IL-24 has classical immune-modulating properties .
	manualset3
102630	5	401421	13	NULL	NULL	0	NULL	IL-22R	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , immune cells do not appear to express specific IL-24 receptor chains ( IL-20R1 / IL-20R2 and IL-22R / IL-20R2 ) , it is therefore unlikely that IL-24 has classical immune-modulating properties .
	manualset3
102631	6	401421	13	NULL	NULL	0	NULL	IL-20R2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , immune cells do not appear to express specific IL-24 receptor chains ( IL-20R1 / IL-20R2 and IL-22R / IL-20R2 ) , it is therefore unlikely that IL-24 has classical immune-modulating properties .
	manualset3
102632	7	401421	13	NULL	NULL	0	NULL	IL-24 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , immune cells do not appear to express specific IL-24 receptor chains ( IL-20R1 / IL-20R2 and IL-22R / IL-20R2 ) , it is therefore unlikely that IL-24 has classical immune-modulating properties .
	manualset3
102633	8	401421	13	NULL	NULL	0	NULL	immune-modulating properties	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , immune cells do not appear to express specific IL-24 receptor chains ( IL-20R1 / IL-20R2 and IL-22R / IL-20R2 ) , it is therefore unlikely that IL-24 has classical immune-modulating properties .
	manualset3
102634	1	401422	13	NULL	NULL	0	NULL	lysis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , lysis by all three Abs at high concentrations was mostly complement dependent , because it was blocked by the anti-C5 Ab eculizumab by 90 % in the case of alemtuzumab and rituximab and by 64 % in the case of GA101 .
	manualset3
102635	2	401422	13	NULL	NULL	0	NULL	three Abs 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , lysis by all three Abs at high concentrations was mostly complement dependent , because it was blocked by the anti-C5 Ab eculizumab by 90 % in the case of alemtuzumab and rituximab and by 64 % in the case of GA101 .
	manualset3
102636	3	401422	13	NULL	NULL	0	NULL	concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , lysis by all three Abs at high concentrations was mostly complement dependent , because it was blocked by the anti-C5 Ab eculizumab by 90 % in the case of alemtuzumab and rituximab and by 64 % in the case of GA101 .
	manualset3
102637	4	401422	13	NULL	NULL	0	NULL	anti-C5 Ab eculizumab	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , lysis by all three Abs at high concentrations was mostly complement dependent , because it was blocked by the anti-C5 Ab eculizumab by 90 % in the case of alemtuzumab and rituximab and by 64 % in the case of GA101 .
	manualset3
102638	5	401422	13	NULL	NULL	0	NULL	90 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , lysis by all three Abs at high concentrations was mostly complement dependent , because it was blocked by the anti-C5 Ab eculizumab by 90 % in the case of alemtuzumab and rituximab and by 64 % in the case of GA101 .
	manualset3
102639	6	401422	13	NULL	NULL	0	NULL	case	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , lysis by all three Abs at high concentrations was mostly complement dependent , because it was blocked by the anti-C5 Ab eculizumab by 90 % in the case of alemtuzumab and rituximab and by 64 % in the case of GA101 .
	manualset3
102640	7	401422	13	NULL	NULL	0	NULL	alemtuzumab	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , lysis by all three Abs at high concentrations was mostly complement dependent , because it was blocked by the anti-C5 Ab eculizumab by 90 % in the case of alemtuzumab and rituximab and by 64 % in the case of GA101 .
	manualset3
102641	8	401422	13	NULL	NULL	0	NULL	rituximab	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , lysis by all three Abs at high concentrations was mostly complement dependent , because it was blocked by the anti-C5 Ab eculizumab by 90 % in the case of alemtuzumab and rituximab and by 64 % in the case of GA101 .
	manualset3
102642	9	401422	13	NULL	NULL	0	NULL	64 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , lysis by all three Abs at high concentrations was mostly complement dependent , because it was blocked by the anti-C5 Ab eculizumab by 90 % in the case of alemtuzumab and rituximab and by 64 % in the case of GA101 .
	manualset3
102643	10	401422	13	NULL	NULL	0	NULL	case 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , lysis by all three Abs at high concentrations was mostly complement dependent , because it was blocked by the anti-C5 Ab eculizumab by 90 % in the case of alemtuzumab and rituximab and by 64 % in the case of GA101 .
	manualset3
102644	11	401422	13	NULL	NULL	0	NULL	GA101 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , lysis by all three Abs at high concentrations was mostly complement dependent , because it was blocked by the anti-C5 Ab eculizumab by 90 % in the case of alemtuzumab and rituximab and by 64 % in the case of GA101 .
	manualset3
102645	1	401423	13	NULL	NULL	0	NULL	31P NMR spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	31P NMR spectroscopy was performed on rabbit urinary bladders ( n = 4 ) to characterize insulin 's actions on smooth muscle .
	manualset3
102646	2	401423	13	NULL	NULL	0	NULL	rabbit urinary bladders 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	31P NMR spectroscopy was performed on rabbit urinary bladders ( n = 4 ) to characterize insulin 's actions on smooth muscle .
	manualset3
102647	3	401423	13	NULL	NULL	0	NULL	n = 4	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	31P NMR spectroscopy was performed on rabbit urinary bladders ( n = 4 ) to characterize insulin 's actions on smooth muscle .
	manualset3
102648	4	401423	13	NULL	NULL	0	NULL	 insulin 's actions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	31P NMR spectroscopy was performed on rabbit urinary bladders ( n = 4 ) to characterize insulin 's actions on smooth muscle .
	manualset3
102649	5	401423	13	NULL	NULL	NULL	NULL	smooth muscle	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	31P NMR spectroscopy was performed on rabbit urinary bladders ( n = 4 ) to characterize insulin 's actions on smooth muscle .
	manualset3
102650	1	401424	13	NULL	NULL	0	NULL	sirolimus	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , sirolimus preserved renal epithelial cell expression of E-cadherin in TgS .
	manualset3
102651	2	401424	13	NULL	NULL	0	NULL	renal epithelial cell 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , sirolimus preserved renal epithelial cell expression of E-cadherin in TgS .
	manualset3
102652	3	401424	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , sirolimus preserved renal epithelial cell expression of E-cadherin in TgS .
	manualset3
102653	4	401424	13	NULL	NULL	0	NULL	E-cadherin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , sirolimus preserved renal epithelial cell expression of E-cadherin in TgS .
	manualset3
102663	5	401424	13	NULL	NULL	0	NULL	 TgS 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , sirolimus preserved renal epithelial cell expression of E-cadherin in TgS .
	manualset3
102666	1	401425	13	NULL	NULL	0	NULL	subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , subjects with a fast NAT2 acetylation phenotype tended to have higher levels of DNA adducts .
	manualset3
102670	2	401425	13	NULL	NULL	NULL	NULL	NAT2 acetylation phenotype	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Interestingly , subjects with a fast NAT2 acetylation phenotype tended to have higher levels of DNA adducts .
	manualset3
102672	4	401425	13	NULL	NULL	0	NULL	 levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , subjects with a fast NAT2 acetylation phenotype tended to have higher levels of DNA adducts .
	manualset3
102676	5	401425	13	NULL	NULL	0	NULL	DNA adducts 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , subjects with a fast NAT2 acetylation phenotype tended to have higher levels of DNA adducts .
	manualset3
102678	1	401426	13	NULL	NULL	0	NULL	basal activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , the basal activity of the cAMP-dependent protein kinase A ( PKA ) , a key player in LTM formation , differs in animals with different satiation levels .
	manualset3
102679	2	401426	13	NULL	NULL	0	NULL	cAMP-dependent protein kinase A ( PKA ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , the basal activity of the cAMP-dependent protein kinase A ( PKA ) , a key player in LTM formation , differs in animals with different satiation levels .
	manualset3
102680	3	401426	13	NULL	NULL	0	NULL	key player	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , the basal activity of the cAMP-dependent protein kinase A ( PKA ) , a key player in LTM formation , differs in animals with different satiation levels .
	manualset3
102688	4	401426	13	NULL	NULL	0	NULL	LTM formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , the basal activity of the cAMP-dependent protein kinase A ( PKA ) , a key player in LTM formation , differs in animals with different satiation levels .
	manualset3
102690	5	401426	13	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , the basal activity of the cAMP-dependent protein kinase A ( PKA ) , a key player in LTM formation , differs in animals with different satiation levels .
	manualset3
102692	6	401426	13	NULL	NULL	0	NULL	satiation levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , the basal activity of the cAMP-dependent protein kinase A ( PKA ) , a key player in LTM formation , differs in animals with different satiation levels .
	manualset3
102695	1	401427	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , the results revealed that both short and long naps resulted in similar delayed performance gains .
	manualset3
102697	2	401427	13	NULL	NULL	0	NULL	short naps	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , the results revealed that both short and long naps resulted in similar delayed performance gains .
	manualset3
102698	3	401427	13	NULL	NULL	0	NULL	long naps 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , the results revealed that both short and long naps resulted in similar delayed performance gains .
	manualset3
102699	4	401427	13	NULL	NULL	0	NULL	performance gains	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , the results revealed that both short and long naps resulted in similar delayed performance gains .
	manualset3
102704	1	401428	13	NULL	NULL	0	NULL	inactive enantiomer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , the supposed inactive enantiomer of L-NA , D-NA , also showed an inhibition of brain NOS activity , ranging from 87 to 100 % .
	manualset3
102705	2	401428	13	NULL	NULL	0	NULL	 L-NA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , the supposed inactive enantiomer of L-NA , D-NA , also showed an inhibition of brain NOS activity , ranging from 87 to 100 % .
	manualset3
102707	3	401428	13	NULL	NULL	0	NULL	D-NA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , the supposed inactive enantiomer of L-NA , D-NA , also showed an inhibition of brain NOS activity , ranging from 87 to 100 % .
	manualset3
102708	4	401428	13	NULL	NULL	0	NULL	 inhibition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , the supposed inactive enantiomer of L-NA , D-NA , also showed an inhibition of brain NOS activity , ranging from 87 to 100 % .
	manualset3
102709	5	401428	13	NULL	NULL	0	NULL	brain NOS activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , the supposed inactive enantiomer of L-NA , D-NA , also showed an inhibition of brain NOS activity , ranging from 87 to 100 % .
	manualset3
102710	6	401428	13	NULL	NULL	0	NULL	87 to 100 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , the supposed inactive enantiomer of L-NA , D-NA , also showed an inhibition of brain NOS activity , ranging from 87 to 100 % .
	manualset3
102715	1	401429	13	NULL	NULL	0	NULL	Wp/BHRF1 connection	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , this Wp/BHRF1 connection is not confined to Wp-restricted BLs but appears integral to normal B cell transformation by EBV .
	manualset3
102716	2	401429	13	NULL	NULL	0	NULL	Wp-restricted BLs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , this Wp/BHRF1 connection is not confined to Wp-restricted BLs but appears integral to normal B cell transformation by EBV .
	manualset3
102717	3	401429	13	NULL	NULL	0	NULL	integral 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , this Wp/BHRF1 connection is not confined to Wp-restricted BLs but appears integral to normal B cell transformation by EBV .
	manualset3
102718	4	401429	13	NULL	NULL	0	NULL	 normal B cell transformation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , this Wp/BHRF1 connection is not confined to Wp-restricted BLs but appears integral to normal B cell transformation by EBV .
	manualset3
102719	5	401429	13	NULL	NULL	0	NULL	EBV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , this Wp/BHRF1 connection is not confined to Wp-restricted BLs but appears integral to normal B cell transformation by EBV .
	manualset3
102720	1	401430	13	NULL	NULL	0	NULL	PFC	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , we found that these various PFC and related areas strongly contribute to active consciousness based on the working memory system .
	manualset3
102721	2	401430	13	NULL	NULL	0	NULL	areas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , we found that these various PFC and related areas strongly contribute to active consciousness based on the working memory system .
	manualset3
102722	3	401430	13	NULL	NULL	0	NULL	active consciousness 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , we found that these various PFC and related areas strongly contribute to active consciousness based on the working memory system .
	manualset3
102724	4	401430	13	NULL	NULL	NULL	NULL	working memory system 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Interestingly , we found that these various PFC and related areas strongly contribute to active consciousness based on the working memory system .
	manualset3
102750	1	401431	13	NULL	NULL	0	NULL	rabies virus glycoprotein mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , we observed that the rabies virus glycoprotein mRNA is differentially over-expressed based on this model relative to other transcripts during infection of 293T cells .
	manualset3
102759	2	401431	13	NULL	NULL	NULL	NULL	model	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Interestingly , we observed that the rabies virus glycoprotein mRNA is differentially over-expressed based on this model relative to other transcripts during infection of 293T cells .
	manualset3
102761	3	401431	13	NULL	NULL	0	NULL	transcripts 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , we observed that the rabies virus glycoprotein mRNA is differentially over-expressed based on this model relative to other transcripts during infection of 293T cells .
	manualset3
102763	4	401431	13	NULL	NULL	NULL	NULL	 infection 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Interestingly , we observed that the rabies virus glycoprotein mRNA is differentially over-expressed based on this model relative to other transcripts during infection of 293T cells .
	manualset3
102766	5	401431	13	NULL	NULL	0	NULL	293T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , we observed that the rabies virus glycoprotein mRNA is differentially over-expressed based on this model relative to other transcripts during infection of 293T cells .
	manualset3
102767	1	401432	13	NULL	NULL	0	NULL	37	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	37 patients were 44 times treated with cotrimoxazole for an infection of the urinary tract during a renal insufficiency .
	manualset3
102768	2	401432	13	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	37 patients were 44 times treated with cotrimoxazole for an infection of the urinary tract during a renal insufficiency .
	manualset3
102769	3	401432	13	NULL	NULL	0	NULL	44 times 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	37 patients were 44 times treated with cotrimoxazole for an infection of the urinary tract during a renal insufficiency .
	manualset3
102770	4	401432	13	NULL	NULL	0	NULL	cotrimoxazole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	37 patients were 44 times treated with cotrimoxazole for an infection of the urinary tract during a renal insufficiency .
	manualset3
102771	5	401432	13	NULL	NULL	0	NULL	infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	37 patients were 44 times treated with cotrimoxazole for an infection of the urinary tract during a renal insufficiency .
	manualset3
102772	6	401432	13	NULL	NULL	0	NULL	urinary tract 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	37 patients were 44 times treated with cotrimoxazole for an infection of the urinary tract during a renal insufficiency .
	manualset3
102773	7	401432	13	NULL	NULL	0	NULL	renal insufficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	37 patients were 44 times treated with cotrimoxazole for an infection of the urinary tract during a renal insufficiency .
	manualset3
102777	1	401433	13	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , we showed that in addition to RBPs , poly ( A ) + RNA is also accumulated into the nucleolus in response to ActD treatment .
	manualset3
102778	2	401433	13	NULL	NULL	0	NULL	 RBPs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , we showed that in addition to RBPs , poly ( A ) + RNA is also accumulated into the nucleolus in response to ActD treatment .
	manualset3
102779	3	401433	13	NULL	NULL	0	NULL	poly ( A ) + RNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , we showed that in addition to RBPs , poly ( A ) + RNA is also accumulated into the nucleolus in response to ActD treatment .
	manualset3
102780	4	401433	13	NULL	NULL	0	NULL	nucleolus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , we showed that in addition to RBPs , poly ( A ) + RNA is also accumulated into the nucleolus in response to ActD treatment .
	manualset3
102785	6	401433	13	NULL	NULL	0	NULL	ActD 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , we showed that in addition to RBPs , poly ( A ) + RNA is also accumulated into the nucleolus in response to ActD treatment .
	manualset3
102787	7	401433	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , we showed that in addition to RBPs , poly ( A ) + RNA is also accumulated into the nucleolus in response to ActD treatment .
	manualset3
102795	1	401434	13	NULL	NULL	0	NULL	Interfacial pH	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Interfacial pH at an isolated silica-water surface .
	manualset3
102799	2	401434	13	NULL	NULL	0	NULL	silica-water surface	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Interfacial pH at an isolated silica-water surface .
	manualset3
102801	1	401435	13	NULL	NULL	0	NULL	Interferents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferents , such as ascorbic acid , were separated from the analyte electrophoretically , so that glucose could be quantified in diluted juices .
	manualset3
102802	2	401435	13	NULL	NULL	0	NULL	ascorbic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferents , such as ascorbic acid , were separated from the analyte electrophoretically , so that glucose could be quantified in diluted juices .
	manualset3
102803	3	401435	13	NULL	NULL	0	NULL	analyte	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferents , such as ascorbic acid , were separated from the analyte electrophoretically , so that glucose could be quantified in diluted juices .
	manualset3
102804	4	401435	13	NULL	NULL	0	NULL	glucose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferents , such as ascorbic acid , were separated from the analyte electrophoretically , so that glucose could be quantified in diluted juices .
	manualset3
102809	5	401435	13	NULL	NULL	0	NULL	juices	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferents , such as ascorbic acid , were separated from the analyte electrophoretically , so that glucose could be quantified in diluted juices .
	manualset3
102810	1	401436	13	NULL	NULL	0	NULL	Interferon-gamma-induced conversion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferon-gamma-induced conversion of tryptophan : immunologic and neuropsychiatric aspects .
	manualset3
102811	2	401436	13	NULL	NULL	0	NULL	tryptophan	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferon-gamma-induced conversion of tryptophan : immunologic and neuropsychiatric aspects .
	manualset3
102812	3	401436	13	NULL	NULL	0	NULL	immunologic aspects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferon-gamma-induced conversion of tryptophan : immunologic and neuropsychiatric aspects .
	manualset3
102813	4	401436	13	NULL	NULL	0	NULL	neuropsychiatric aspects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferon-gamma-induced conversion of tryptophan : immunologic and neuropsychiatric aspects .
	manualset3
102814	1	401437	13	NULL	NULL	0	NULL	Interferon-gamma	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferon-gamma co-treatment increased the stability of p53 protein induced by adriamycin .
	manualset3
102815	2	401437	13	NULL	NULL	0	NULL	co-treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferon-gamma co-treatment increased the stability of p53 protein induced by adriamycin .
	manualset3
102816	3	401437	13	NULL	NULL	0	NULL	 stability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferon-gamma co-treatment increased the stability of p53 protein induced by adriamycin .
	manualset3
102817	4	401437	13	NULL	NULL	0	NULL	p53 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferon-gamma co-treatment increased the stability of p53 protein induced by adriamycin .
	manualset3
102818	5	401437	13	NULL	NULL	0	NULL	adriamycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferon-gamma co-treatment increased the stability of p53 protein induced by adriamycin .
	manualset3
102819	1	401438	13	NULL	NULL	0	NULL	Interferon - release assays 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferon - release assays for the diagnosis of latent Mycobacterium tuberculosis infection : a systematic review and meta-analysis .
	manualset3
102820	2	401438	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferon - release assays for the diagnosis of latent Mycobacterium tuberculosis infection : a systematic review and meta-analysis .
	manualset3
102821	3	401438	13	NULL	NULL	0	NULL	 latent Mycobacterium tuberculosis infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferon - release assays for the diagnosis of latent Mycobacterium tuberculosis infection : a systematic review and meta-analysis .
	manualset3
102822	4	401438	13	NULL	NULL	0	NULL	a systematic review	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferon - release assays for the diagnosis of latent Mycobacterium tuberculosis infection : a systematic review and meta-analysis .
	manualset3
102823	5	401438	13	NULL	NULL	0	NULL	meta-analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferon - release assays for the diagnosis of latent Mycobacterium tuberculosis infection : a systematic review and meta-analysis .
	manualset3
102824	1	401439	13	NULL	NULL	0	NULL	Interferon gamma	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferon gamma bound to endothelial cells is phosphorylated by ecto-protein kinases .
	manualset3
102825	2	401439	13	NULL	NULL	0	NULL	endothelial cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferon gamma bound to endothelial cells is phosphorylated by ecto-protein kinases .
	manualset3
102826	3	401439	13	NULL	NULL	0	NULL	ecto-protein kinases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferon gamma bound to endothelial cells is phosphorylated by ecto-protein kinases .
	manualset3
102827	1	401440	13	NULL	NULL	0	NULL	Interferon regulatory factor 5 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferon regulatory factor 5 is critical for the development of lupus in MRL/lpr mice .
	manualset3
102828	2	401440	13	NULL	NULL	0	NULL	development of lupus 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferon regulatory factor 5 is critical for the development of lupus in MRL/lpr mice .
	manualset3
102829	3	401440	13	NULL	NULL	0	NULL	MRL/lpr mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferon regulatory factor 5 is critical for the development of lupus in MRL/lpr mice .
	manualset3
102830	1	401441	13	NULL	NULL	0	NULL	Interictal myoclonus	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interictal myoclonus could be a manifestation of permanent overexcitability .
	manualset3
102831	2	401441	13	NULL	NULL	0	NULL	manifestation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interictal myoclonus could be a manifestation of permanent overexcitability .
	manualset3
102832	3	401441	13	NULL	NULL	0	NULL	overexcitability 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interictal myoclonus could be a manifestation of permanent overexcitability .
	manualset3
102833	1	401442	13	NULL	NULL	0	NULL	Interleukin-1 beta 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-1 beta induces the synthesis and activity of cytosolic phospholipase A2 and the release of prostaglandin E2 in human amnion-derived WISH cells .
	manualset3
102834	2	401442	13	NULL	NULL	0	NULL	synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-1 beta induces the synthesis and activity of cytosolic phospholipase A2 and the release of prostaglandin E2 in human amnion-derived WISH cells .
	manualset3
102835	3	401442	13	NULL	NULL	0	NULL	activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-1 beta induces the synthesis and activity of cytosolic phospholipase A2 and the release of prostaglandin E2 in human amnion-derived WISH cells .
	manualset3
102836	4	401442	13	NULL	NULL	0	NULL	 cytosolic phospholipase A2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-1 beta induces the synthesis and activity of cytosolic phospholipase A2 and the release of prostaglandin E2 in human amnion-derived WISH cells .
	manualset3
102837	5	401442	13	NULL	NULL	0	NULL	release of prostaglandin E2 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-1 beta induces the synthesis and activity of cytosolic phospholipase A2 and the release of prostaglandin E2 in human amnion-derived WISH cells .
	manualset3
102838	6	401442	13	NULL	NULL	0	NULL	human amnion-derived WISH cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-1 beta induces the synthesis and activity of cytosolic phospholipase A2 and the release of prostaglandin E2 in human amnion-derived WISH cells .
	manualset3
102839	1	401443	13	NULL	NULL	NULL	NULL	Interleukin-12	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Interleukin-12 enhancement of antigen-specific lymphocyte proliferation correlates with stage of human immunodeficiency virus infection .
	manualset3
102840	2	401443	13	NULL	NULL	0	NULL	enhancement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-12 enhancement of antigen-specific lymphocyte proliferation correlates with stage of human immunodeficiency virus infection .
	manualset3
102841	3	401443	13	NULL	NULL	0	NULL	antigen-specific lymphocyte proliferation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-12 enhancement of antigen-specific lymphocyte proliferation correlates with stage of human immunodeficiency virus infection .
	manualset3
102842	4	401443	13	NULL	NULL	0	NULL	stage of human immunodeficiency virus infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-12 enhancement of antigen-specific lymphocyte proliferation correlates with stage of human immunodeficiency virus infection .
	manualset3
102843	1	401444	13	NULL	NULL	0	NULL	Interleukin-32	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-32 , CCL2 , PF4F1 and GFD10 are the only cytokine/chemokine genes differentially expressed by in vitro cultured rheumatoid and osteoarthritis fibroblast-like synoviocytes .
	manualset3
102844	2	401444	13	NULL	NULL	0	NULL	CCL2	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-32 , CCL2 , PF4F1 and GFD10 are the only cytokine/chemokine genes differentially expressed by in vitro cultured rheumatoid and osteoarthritis fibroblast-like synoviocytes .
	manualset3
102845	3	401444	13	NULL	NULL	0	NULL	PF4F1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-32 , CCL2 , PF4F1 and GFD10 are the only cytokine/chemokine genes differentially expressed by in vitro cultured rheumatoid and osteoarthritis fibroblast-like synoviocytes .
	manualset3
102846	4	401444	13	NULL	NULL	0	NULL	GFD10 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-32 , CCL2 , PF4F1 and GFD10 are the only cytokine/chemokine genes differentially expressed by in vitro cultured rheumatoid and osteoarthritis fibroblast-like synoviocytes .
	manualset3
102847	5	401444	13	NULL	NULL	0	NULL	cytokine/chemokine genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-32 , CCL2 , PF4F1 and GFD10 are the only cytokine/chemokine genes differentially expressed by in vitro cultured rheumatoid and osteoarthritis fibroblast-like synoviocytes .
	manualset3
102848	6	401444	13	NULL	NULL	0	NULL	cultured rheumatoid fibroblast-like synoviocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-32 , CCL2 , PF4F1 and GFD10 are the only cytokine/chemokine genes differentially expressed by in vitro cultured rheumatoid and osteoarthritis fibroblast-like synoviocytes .
	manualset3
102849	7	401444	13	NULL	NULL	0	NULL	cultured osteoarthritis fibroblast-like synoviocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-32 , CCL2 , PF4F1 and GFD10 are the only cytokine/chemokine genes differentially expressed by in vitro cultured rheumatoid and osteoarthritis fibroblast-like synoviocytes .
	manualset3
102850	1	401445	13	NULL	NULL	0	NULL	Interleukin-6 ( IL-6 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-6 ( IL-6 ) , mainly secreted by activated monocytes/macrophages , is also an early prognostic parameter ( shown in one study ) , but is not superior to PMN-elastase .
	manualset3
102851	2	401445	13	NULL	NULL	0	NULL	monocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-6 ( IL-6 ) , mainly secreted by activated monocytes/macrophages , is also an early prognostic parameter ( shown in one study ) , but is not superior to PMN-elastase .
	manualset3
102852	3	401445	13	NULL	NULL	0	NULL	macrophages 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-6 ( IL-6 ) , mainly secreted by activated monocytes/macrophages , is also an early prognostic parameter ( shown in one study ) , but is not superior to PMN-elastase .
	manualset3
102853	4	401445	13	NULL	NULL	0	NULL	prognostic parameter	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-6 ( IL-6 ) , mainly secreted by activated monocytes/macrophages , is also an early prognostic parameter ( shown in one study ) , but is not superior to PMN-elastase .
	manualset3
102854	5	401445	13	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-6 ( IL-6 ) , mainly secreted by activated monocytes/macrophages , is also an early prognostic parameter ( shown in one study ) , but is not superior to PMN-elastase .
	manualset3
102855	6	401445	13	NULL	NULL	0	NULL	PMN-elastase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-6 ( IL-6 ) , mainly secreted by activated monocytes/macrophages , is also an early prognostic parameter ( shown in one study ) , but is not superior to PMN-elastase .
	manualset3
102857	1	401446	13	NULL	NULL	0	NULL	Interleukin ( IL ) -17 - producing CD4 ( + ) T lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin ( IL ) -17 - producing CD4 ( + ) T lymphocytes ( T ( H ) 17 cells ) constitute a subset of T-helper cells involved in host defense and several immune disorders .
	manualset3
102858	2	401446	13	NULL	NULL	0	NULL	T ( H ) 17 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin ( IL ) -17 - producing CD4 ( + ) T lymphocytes ( T ( H ) 17 cells ) constitute a subset of T-helper cells involved in host defense and several immune disorders .
	manualset3
102859	3	401446	13	NULL	NULL	0	NULL	subset of T-helper cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin ( IL ) -17 - producing CD4 ( + ) T lymphocytes ( T ( H ) 17 cells ) constitute a subset of T-helper cells involved in host defense and several immune disorders .
	manualset3
102860	4	401446	13	NULL	NULL	0	NULL	host defense 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin ( IL ) -17 - producing CD4 ( + ) T lymphocytes ( T ( H ) 17 cells ) constitute a subset of T-helper cells involved in host defense and several immune disorders .
	manualset3
102861	5	401446	13	NULL	NULL	0	NULL	several immune disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin ( IL ) -17 - producing CD4 ( + ) T lymphocytes ( T ( H ) 17 cells ) constitute a subset of T-helper cells involved in host defense and several immune disorders .
	manualset3
102862	1	401447	13	NULL	NULL	0	NULL	Interleukin ( IL ) -4 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin ( IL ) -4 is a central regulator of T helper 2 ( Th2 ) immune responses , and also has a major impact on innate immune cells .
	manualset3
102863	2	401447	13	NULL	NULL	0	NULL	central regulator	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin ( IL ) -4 is a central regulator of T helper 2 ( Th2 ) immune responses , and also has a major impact on innate immune cells .
	manualset3
102864	3	401447	13	NULL	NULL	0	NULL	T helper 2 ( Th2 ) immune responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin ( IL ) -4 is a central regulator of T helper 2 ( Th2 ) immune responses , and also has a major impact on innate immune cells .
	manualset3
102865	4	401447	13	NULL	NULL	0	NULL	impact 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin ( IL ) -4 is a central regulator of T helper 2 ( Th2 ) immune responses , and also has a major impact on innate immune cells .
	manualset3
102866	5	401447	13	NULL	NULL	0	NULL	innate immune cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin ( IL ) -4 is a central regulator of T helper 2 ( Th2 ) immune responses , and also has a major impact on innate immune cells .
	manualset3
102867	1	401448	13	NULL	NULL	0	NULL	Interleukin 2 responsive T cell clones	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin 2 responsive T cell clones from rheumatoid and normal subjects : proliferative responses to connective tissue elements .
	manualset3
102868	2	401448	13	NULL	NULL	0	NULL	rheumatoid subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin 2 responsive T cell clones from rheumatoid and normal subjects : proliferative responses to connective tissue elements .
	manualset3
102869	3	401448	13	NULL	NULL	0	NULL	normal subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin 2 responsive T cell clones from rheumatoid and normal subjects : proliferative responses to connective tissue elements .
	manualset3
102870	4	401448	13	NULL	NULL	0	NULL	proliferative responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin 2 responsive T cell clones from rheumatoid and normal subjects : proliferative responses to connective tissue elements .
	manualset3
102871	5	401448	13	NULL	NULL	0	NULL	connective tissue elements	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin 2 responsive T cell clones from rheumatoid and normal subjects : proliferative responses to connective tissue elements .
	manualset3
102879	1	401449	13	NULL	NULL	0	NULL	Intermediate filaments	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Intermediate filaments have long been considered mechanical components of the cell that provide resistance to deformation stress .
	manualset3
102880	2	401449	13	NULL	NULL	0	NULL	mechanical components	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Intermediate filaments have long been considered mechanical components of the cell that provide resistance to deformation stress .
	manualset3
102881	3	401449	13	NULL	NULL	0	NULL	cell 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Intermediate filaments have long been considered mechanical components of the cell that provide resistance to deformation stress .
	manualset3
102882	4	401449	13	NULL	NULL	0	NULL	resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intermediate filaments have long been considered mechanical components of the cell that provide resistance to deformation stress .
	manualset3
102883	5	401449	13	NULL	NULL	0	NULL	deformation stress 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intermediate filaments have long been considered mechanical components of the cell that provide resistance to deformation stress .
	manualset3
102885	1	401450	13	NULL	NULL	0	NULL	Intermittent injections	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intermittent injections of factor concentrate were given every 12 for 48 h. While the first two doses were given at higher amount to achieve or continue plasma factor level at 90-100 % , in the last three doses , the aim was to maintain the plasma factor level at 50-60 % .
	manualset3
102886	2	401450	13	NULL	NULL	0	NULL	factor concentrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Intermittent injections of factor concentrate were given every 12 for 48 h. While the first two doses were given at higher amount to achieve or continue plasma factor level at 90-100 % , in the last three doses , the aim was to maintain the plasma factor level at 50-60 % .
	manualset3
102887	3	401450	13	NULL	NULL	0	NULL	 12 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Intermittent injections of factor concentrate were given every 12 for 48 h. While the first two doses were given at higher amount to achieve or continue plasma factor level at 90-100 % , in the last three doses , the aim was to maintain the plasma factor level at 50-60 % .
	manualset3
102888	4	401450	13	NULL	NULL	0	NULL	48 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Intermittent injections of factor concentrate were given every 12 for 48 h. While the first two doses were given at higher amount to achieve or continue plasma factor level at 90-100 % , in the last three doses , the aim was to maintain the plasma factor level at 50-60 % .
	manualset3
102889	5	401450	13	NULL	NULL	0	NULL	two doses	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intermittent injections of factor concentrate were given every 12 for 48 h. While the first two doses were given at higher amount to achieve or continue plasma factor level at 90-100 % , in the last three doses , the aim was to maintain the plasma factor level at 50-60 % .
	manualset3
102890	6	401450	13	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Intermittent injections of factor concentrate were given every 12 for 48 h. While the first two doses were given at higher amount to achieve or continue plasma factor level at 90-100 % , in the last three doses , the aim was to maintain the plasma factor level at 50-60 % .
	manualset3
102891	7	401450	13	NULL	NULL	0	NULL	plasma factor level	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intermittent injections of factor concentrate were given every 12 for 48 h. While the first two doses were given at higher amount to achieve or continue plasma factor level at 90-100 % , in the last three doses , the aim was to maintain the plasma factor level at 50-60 % .
	manualset3
102892	8	401450	13	NULL	NULL	0	NULL	 90-100 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intermittent injections of factor concentrate were given every 12 for 48 h. While the first two doses were given at higher amount to achieve or continue plasma factor level at 90-100 % , in the last three doses , the aim was to maintain the plasma factor level at 50-60 % .
	manualset3
102893	9	401450	13	NULL	NULL	0	NULL	last three doses	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intermittent injections of factor concentrate were given every 12 for 48 h. While the first two doses were given at higher amount to achieve or continue plasma factor level at 90-100 % , in the last three doses , the aim was to maintain the plasma factor level at 50-60 % .
	manualset3
102894	10	401450	13	NULL	NULL	0	NULL	aim	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Intermittent injections of factor concentrate were given every 12 for 48 h. While the first two doses were given at higher amount to achieve or continue plasma factor level at 90-100 % , in the last three doses , the aim was to maintain the plasma factor level at 50-60 % .
	manualset3
102895	11	401450	13	NULL	NULL	0	NULL	plasma factor level	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intermittent injections of factor concentrate were given every 12 for 48 h. While the first two doses were given at higher amount to achieve or continue plasma factor level at 90-100 % , in the last three doses , the aim was to maintain the plasma factor level at 50-60 % .
	manualset3
102896	12	401450	13	NULL	NULL	0	NULL	 50-60 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intermittent injections of factor concentrate were given every 12 for 48 h. While the first two doses were given at higher amount to achieve or continue plasma factor level at 90-100 % , in the last three doses , the aim was to maintain the plasma factor level at 50-60 % .
	manualset3
102897	1	401451	13	NULL	NULL	0	NULL	Internal carotid artery ( ICA ) agenesis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Internal carotid artery ( ICA ) agenesis is a rare developmental anomaly and is most frequently asymptomatic , but it may also present as cerebrovascular accidents .
	manualset3
102898	2	401451	13	NULL	NULL	0	NULL	developmental anomaly	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Internal carotid artery ( ICA ) agenesis is a rare developmental anomaly and is most frequently asymptomatic , but it may also present as cerebrovascular accidents .
	manualset3
102899	3	401451	13	NULL	NULL	0	NULL	 cerebrovascular accidents 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Internal carotid artery ( ICA ) agenesis is a rare developmental anomaly and is most frequently asymptomatic , but it may also present as cerebrovascular accidents .
	manualset3
102900	1	401452	13	NULL	NULL	0	NULL	3D Echo	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	3D Echo systematically underestimates right ventricular volumes compared to cardiovascular magnetic resonance in adult congenital heart disease patients with moderate or severe RV dilatation .
	manualset3
102901	2	401452	13	NULL	NULL	0	NULL	right ventricular volumes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	3D Echo systematically underestimates right ventricular volumes compared to cardiovascular magnetic resonance in adult congenital heart disease patients with moderate or severe RV dilatation .
	manualset3
102902	3	401452	13	NULL	NULL	0	NULL	cardiovascular magnetic resonance	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	3D Echo systematically underestimates right ventricular volumes compared to cardiovascular magnetic resonance in adult congenital heart disease patients with moderate or severe RV dilatation .
	manualset3
102903	4	401452	13	NULL	NULL	0	NULL	adult congenital heart disease patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	3D Echo systematically underestimates right ventricular volumes compared to cardiovascular magnetic resonance in adult congenital heart disease patients with moderate or severe RV dilatation .
	manualset3
102904	5	401452	13	NULL	NULL	0	NULL	 moderate RV dilatation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	3D Echo systematically underestimates right ventricular volumes compared to cardiovascular magnetic resonance in adult congenital heart disease patients with moderate or severe RV dilatation .
	manualset3
102905	6	401452	13	NULL	NULL	0	NULL	severe RV dilatation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	3D Echo systematically underestimates right ventricular volumes compared to cardiovascular magnetic resonance in adult congenital heart disease patients with moderate or severe RV dilatation .
	manualset3
102906	1	401453	13	NULL	NULL	0	NULL	Internal carotid artery occlusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Internal carotid artery occlusion assessed at pulsed arterial spin-labeling perfusion MR imaging at multiple delay times .
	manualset3
102907	2	401453	13	NULL	NULL	NULL	NULL	pulsed arterial spin-labeling 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Internal carotid artery occlusion assessed at pulsed arterial spin-labeling perfusion MR imaging at multiple delay times .
	manualset3
102908	4	401453	13	NULL	NULL	NULL	NULL	 multiple delay times	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Internal carotid artery occlusion assessed at pulsed arterial spin-labeling perfusion MR imaging at multiple delay times .
	manualset3
102909	3	401453	13	NULL	NULL	0	NULL	perfusion MR imaging 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Internal carotid artery occlusion assessed at pulsed arterial spin-labeling perfusion MR imaging at multiple delay times .
	manualset3
102910	1	401454	13	NULL	NULL	0	NULL	Internal gas analyzer	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Internal gas analyzer leak resulting in an abnormal capnogram and incorrect calibration .
	manualset3
102911	2	401454	13	NULL	NULL	0	NULL	 leak 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Internal gas analyzer leak resulting in an abnormal capnogram and incorrect calibration .
	manualset3
102912	3	401454	13	NULL	NULL	NULL	NULL	abnormal capnogram	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Internal gas analyzer leak resulting in an abnormal capnogram and incorrect calibration .
	manualset3
102913	4	401454	13	NULL	NULL	0	NULL	calibration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Internal gas analyzer leak resulting in an abnormal capnogram and incorrect calibration .
	manualset3
102914	1	401455	13	NULL	NULL	0	NULL	Internal structural organization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Internal structural organization of chloroplast DNA from Euglena gracilis Z .
	manualset3
102915	2	401455	13	NULL	NULL	0	NULL	chloroplast DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Internal structural organization of chloroplast DNA from Euglena gracilis Z .
	manualset3
102916	3	401455	13	NULL	NULL	0	NULL	Euglena gracilis Z	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Internal structural organization of chloroplast DNA from Euglena gracilis Z .
	manualset3
102917	1	401456	13	NULL	NULL	0	NULL	Internal IT support 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Internal IT support crucial to success in filmless department .
	manualset3
102918	2	401456	13	NULL	NULL	0	NULL	success	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Internal IT support crucial to success in filmless department .
	manualset3
102919	3	401456	13	NULL	NULL	0	NULL	filmless department	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Internal IT support crucial to success in filmless department .
	manualset3
102920	1	401457	13	NULL	NULL	0	NULL	Internalin B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Internalin B is essential for adhesion and mediates the invasion of Listeria monocytogenes into human endothelial cells .
	manualset3
102921	2	401457	13	NULL	NULL	0	NULL	adhesion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Internalin B is essential for adhesion and mediates the invasion of Listeria monocytogenes into human endothelial cells .
	manualset3
102922	3	401457	13	NULL	NULL	0	NULL	invasion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Internalin B is essential for adhesion and mediates the invasion of Listeria monocytogenes into human endothelial cells .
	manualset3
102923	4	401457	13	NULL	NULL	0	NULL	Listeria monocytogenes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Internalin B is essential for adhesion and mediates the invasion of Listeria monocytogenes into human endothelial cells .
	manualset3
102924	5	401457	13	NULL	NULL	0	NULL	human endothelial cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Internalin B is essential for adhesion and mediates the invasion of Listeria monocytogenes into human endothelial cells .
	manualset3
102925	1	401458	13	NULL	NULL	0	NULL	JTat	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Internalized JTat was distributed in both the nucleus and the cytoplasm , could transactivate JDV LTR and modulate cellular gene expression .
	manualset3
102926	2	401458	13	NULL	NULL	0	NULL	 nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Internalized JTat was distributed in both the nucleus and the cytoplasm , could transactivate JDV LTR and modulate cellular gene expression .
	manualset3
102927	3	401458	13	NULL	NULL	0	NULL	 cytoplasm	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Internalized JTat was distributed in both the nucleus and the cytoplasm , could transactivate JDV LTR and modulate cellular gene expression .
	manualset3
102928	4	401458	13	NULL	NULL	0	NULL	JDV LTR 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Internalized JTat was distributed in both the nucleus and the cytoplasm , could transactivate JDV LTR and modulate cellular gene expression .
	manualset3
102929	5	401458	13	NULL	NULL	0	NULL	cellular gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Internalized JTat was distributed in both the nucleus and the cytoplasm , could transactivate JDV LTR and modulate cellular gene expression .
	manualset3
102930	1	401459	13	NULL	NULL	0	NULL	proactive individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Internally oriented , proactive individuals perceive their jobs to be more enriched and intrinsically motivating than externally oriented , reactive individuals who report low levels of job satisfaction and higher levels of perceived powerlessness .
	manualset3
102931	2	401459	13	NULL	NULL	0	NULL	jobs	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Internally oriented , proactive individuals perceive their jobs to be more enriched and intrinsically motivating than externally oriented , reactive individuals who report low levels of job satisfaction and higher levels of perceived powerlessness .
	manualset3
102932	3	401459	13	NULL	NULL	0	NULL	reactive individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Internally oriented , proactive individuals perceive their jobs to be more enriched and intrinsically motivating than externally oriented , reactive individuals who report low levels of job satisfaction and higher levels of perceived powerlessness .
	manualset3
102933	4	401459	13	NULL	NULL	0	NULL	low levels 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Internally oriented , proactive individuals perceive their jobs to be more enriched and intrinsically motivating than externally oriented , reactive individuals who report low levels of job satisfaction and higher levels of perceived powerlessness .
	manualset3
102934	5	401459	13	NULL	NULL	0	NULL	job satisfaction	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Internally oriented , proactive individuals perceive their jobs to be more enriched and intrinsically motivating than externally oriented , reactive individuals who report low levels of job satisfaction and higher levels of perceived powerlessness .
	manualset3
102935	6	401459	13	NULL	NULL	0	NULL	higher levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Internally oriented , proactive individuals perceive their jobs to be more enriched and intrinsically motivating than externally oriented , reactive individuals who report low levels of job satisfaction and higher levels of perceived powerlessness .
	manualset3
102936	7	401459	13	NULL	NULL	0	NULL	powerlessness	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Internally oriented , proactive individuals perceive their jobs to be more enriched and intrinsically motivating than externally oriented , reactive individuals who report low levels of job satisfaction and higher levels of perceived powerlessness .
	manualset3
102937	1	401460	13	NULL	NULL	0	NULL	Interpeptide interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interpeptide interactions in Abeta dimers and , especially , in the peptides bound to the fibril induce a dramatic shift in the secondary structure , from helical states toward beta-strand conformations .
	manualset3
102938	2	401460	13	NULL	NULL	0	NULL	Abeta dimers	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Interpeptide interactions in Abeta dimers and , especially , in the peptides bound to the fibril induce a dramatic shift in the secondary structure , from helical states toward beta-strand conformations .
	manualset3
102939	3	401460	13	NULL	NULL	0	NULL	peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Interpeptide interactions in Abeta dimers and , especially , in the peptides bound to the fibril induce a dramatic shift in the secondary structure , from helical states toward beta-strand conformations .
	manualset3
102940	4	401460	13	NULL	NULL	NULL	NULL	fibril	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Interpeptide interactions in Abeta dimers and , especially , in the peptides bound to the fibril induce a dramatic shift in the secondary structure , from helical states toward beta-strand conformations .
	manualset3
102941	5	401460	13	NULL	NULL	0	NULL	dramatic shift 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interpeptide interactions in Abeta dimers and , especially , in the peptides bound to the fibril induce a dramatic shift in the secondary structure , from helical states toward beta-strand conformations .
	manualset3
102942	6	401460	13	NULL	NULL	0	NULL	secondary structure	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interpeptide interactions in Abeta dimers and , especially , in the peptides bound to the fibril induce a dramatic shift in the secondary structure , from helical states toward beta-strand conformations .
	manualset3
102943	7	401460	13	NULL	NULL	0	NULL	helical states	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interpeptide interactions in Abeta dimers and , especially , in the peptides bound to the fibril induce a dramatic shift in the secondary structure , from helical states toward beta-strand conformations .
	manualset3
102944	8	401460	13	NULL	NULL	0	NULL	beta-strand conformations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interpeptide interactions in Abeta dimers and , especially , in the peptides bound to the fibril induce a dramatic shift in the secondary structure , from helical states toward beta-strand conformations .
	manualset3
102945	1	401461	13	NULL	NULL	0	NULL	Interplay	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interplay between subsurface ordering , surface segregation , and adsorption on Pt-Ti ( 111 ) near-surface alloys .
	manualset3
102946	2	401461	13	NULL	NULL	0	NULL	ubsurface ordering	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interplay between subsurface ordering , surface segregation , and adsorption on Pt-Ti ( 111 ) near-surface alloys .
	manualset3
102947	3	401461	13	NULL	NULL	0	NULL	surface segregation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interplay between subsurface ordering , surface segregation , and adsorption on Pt-Ti ( 111 ) near-surface alloys .
	manualset3
102948	4	401461	13	NULL	NULL	0	NULL	adsorption 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interplay between subsurface ordering , surface segregation , and adsorption on Pt-Ti ( 111 ) near-surface alloys .
	manualset3
102949	5	401461	13	NULL	NULL	0	NULL	Pt-Ti ( 111 ) near-surface alloys 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Interplay between subsurface ordering , surface segregation , and adsorption on Pt-Ti ( 111 ) near-surface alloys .
	manualset3
102950	1	401462	13	NULL	NULL	0	NULL	Interpretation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Interpretation The RSA analysis for the OPRA system indicated stable fixation of the implant .
	manualset3
102951	2	401462	13	NULL	NULL	0	NULL	RSA analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Interpretation The RSA analysis for the OPRA system indicated stable fixation of the implant .
	manualset3
102952	3	401462	13	NULL	NULL	0	NULL	OPRA system	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Interpretation The RSA analysis for the OPRA system indicated stable fixation of the implant .
	manualset3
102953	4	401462	13	NULL	NULL	0	NULL	stable fixation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Interpretation The RSA analysis for the OPRA system indicated stable fixation of the implant .
	manualset3
102954	5	401462	13	NULL	NULL	0	NULL	implant	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Interpretation The RSA analysis for the OPRA system indicated stable fixation of the implant .
	manualset3
102955	1	401463	13	NULL	NULL	0	NULL	Interpretation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interpretation of these features provides effective guidance in the process of searching , reading and assessing the relevance of different items of information in the record .
	manualset3
102956	2	401463	13	NULL	NULL	0	NULL	features	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Interpretation of these features provides effective guidance in the process of searching , reading and assessing the relevance of different items of information in the record .
	manualset3
102957	3	401463	13	NULL	NULL	0	NULL	effective guidance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interpretation of these features provides effective guidance in the process of searching , reading and assessing the relevance of different items of information in the record .
	manualset3
102958	4	401463	13	NULL	NULL	0	NULL	process of searching	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interpretation of these features provides effective guidance in the process of searching , reading and assessing the relevance of different items of information in the record .
	manualset3
102959	5	401463	13	NULL	NULL	0	NULL	process of reading	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interpretation of these features provides effective guidance in the process of searching , reading and assessing the relevance of different items of information in the record .
	manualset3
102960	6	401463	13	NULL	NULL	0	NULL	process of assessing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interpretation of these features provides effective guidance in the process of searching , reading and assessing the relevance of different items of information in the record .
	manualset3
102961	7	401463	13	NULL	NULL	0	NULL	relevance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interpretation of these features provides effective guidance in the process of searching , reading and assessing the relevance of different items of information in the record .
	manualset3
102962	8	401463	13	NULL	NULL	0	NULL	different items of information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Interpretation of these features provides effective guidance in the process of searching , reading and assessing the relevance of different items of information in the record .
	manualset3
102963	9	401463	13	NULL	NULL	0	NULL	record	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Interpretation of these features provides effective guidance in the process of searching , reading and assessing the relevance of different items of information in the record .
	manualset3
102964	1	401464	13	NULL	NULL	0	NULL	12-lead ECG	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Interpreting the 12-lead ECG for the diagnosis of VT and SVT is a skill that is acquired through practice and the recognition of morphologic clues on the ECG .
	manualset3
102965	2	401464	13	NULL	NULL	0	NULL	diagnosis of VT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Interpreting the 12-lead ECG for the diagnosis of VT and SVT is a skill that is acquired through practice and the recognition of morphologic clues on the ECG .
	manualset3
102966	3	401464	13	NULL	NULL	0	NULL	diagnosis of SVT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Interpreting the 12-lead ECG for the diagnosis of VT and SVT is a skill that is acquired through practice and the recognition of morphologic clues on the ECG .
	manualset3
102967	4	401464	13	NULL	NULL	0	NULL	skill	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Interpreting the 12-lead ECG for the diagnosis of VT and SVT is a skill that is acquired through practice and the recognition of morphologic clues on the ECG .
	manualset3
102968	5	401464	13	NULL	NULL	0	NULL	practice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Interpreting the 12-lead ECG for the diagnosis of VT and SVT is a skill that is acquired through practice and the recognition of morphologic clues on the ECG .
	manualset3
102969	6	401464	13	NULL	NULL	0	NULL	recognition	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Interpreting the 12-lead ECG for the diagnosis of VT and SVT is a skill that is acquired through practice and the recognition of morphologic clues on the ECG .
	manualset3
102970	7	401464	13	NULL	NULL	0	NULL	morphologic clues	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Interpreting the 12-lead ECG for the diagnosis of VT and SVT is a skill that is acquired through practice and the recognition of morphologic clues on the ECG .
	manualset3
102971	8	401464	13	NULL	NULL	0	NULL	ECG 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Interpreting the 12-lead ECG for the diagnosis of VT and SVT is a skill that is acquired through practice and the recognition of morphologic clues on the ECG .
	manualset3
102972	1	401465	13	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Interrupted pregnancy as an indicator of poor prognosis in T1 , 2 , N0 , M0 primary breast cancer .
	manualset3
102973	2	401465	13	NULL	NULL	0	NULL	indicator	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Interrupted pregnancy as an indicator of poor prognosis in T1 , 2 , N0 , M0 primary breast cancer .
	manualset3
102974	3	401465	13	NULL	NULL	0	NULL	prognosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Interrupted pregnancy as an indicator of poor prognosis in T1 , 2 , N0 , M0 primary breast cancer .
	manualset3
102975	4	401465	13	NULL	NULL	0	NULL	T1 , 2 , N0 , M0 primary breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Interrupted pregnancy as an indicator of poor prognosis in T1 , 2 , N0 , M0 primary breast cancer .
	manualset3
102976	1	401466	13	NULL	NULL	0	NULL	Interruption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interruption of tonically active medullo-spinal pathways after injury causes disinhibition of thoracolumbar sympathetic preganglionic neurons , and intraspinal sprouting of nerve growth factor ( NGF ) - responsive primary afferent fibers is thought to contribute to their hyperactivity .
	manualset3
102977	2	401466	13	NULL	NULL	0	NULL	 medullo-spinal pathways	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interruption of tonically active medullo-spinal pathways after injury causes disinhibition of thoracolumbar sympathetic preganglionic neurons , and intraspinal sprouting of nerve growth factor ( NGF ) - responsive primary afferent fibers is thought to contribute to their hyperactivity .
	manualset3
102978	3	401466	13	NULL	NULL	0	NULL	injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Interruption of tonically active medullo-spinal pathways after injury causes disinhibition of thoracolumbar sympathetic preganglionic neurons , and intraspinal sprouting of nerve growth factor ( NGF ) - responsive primary afferent fibers is thought to contribute to their hyperactivity .
	manualset3
102979	4	401466	13	NULL	NULL	0	NULL	causes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Interruption of tonically active medullo-spinal pathways after injury causes disinhibition of thoracolumbar sympathetic preganglionic neurons , and intraspinal sprouting of nerve growth factor ( NGF ) - responsive primary afferent fibers is thought to contribute to their hyperactivity .
	manualset3
102980	5	401466	13	NULL	NULL	0	NULL	thoracolumbar sympathetic preganglionic neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Interruption of tonically active medullo-spinal pathways after injury causes disinhibition of thoracolumbar sympathetic preganglionic neurons , and intraspinal sprouting of nerve growth factor ( NGF ) - responsive primary afferent fibers is thought to contribute to their hyperactivity .
	manualset3
102981	6	401466	13	NULL	NULL	0	NULL	 intraspinal sprouting	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interruption of tonically active medullo-spinal pathways after injury causes disinhibition of thoracolumbar sympathetic preganglionic neurons , and intraspinal sprouting of nerve growth factor ( NGF ) - responsive primary afferent fibers is thought to contribute to their hyperactivity .
	manualset3
102982	7	401466	13	NULL	NULL	0	NULL	nerve growth factor ( NGF ) - responsive primary afferent fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Interruption of tonically active medullo-spinal pathways after injury causes disinhibition of thoracolumbar sympathetic preganglionic neurons , and intraspinal sprouting of nerve growth factor ( NGF ) - responsive primary afferent fibers is thought to contribute to their hyperactivity .
	manualset3
102983	8	401466	13	NULL	NULL	0	NULL	hyperactivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Interruption of tonically active medullo-spinal pathways after injury causes disinhibition of thoracolumbar sympathetic preganglionic neurons , and intraspinal sprouting of nerve growth factor ( NGF ) - responsive primary afferent fibers is thought to contribute to their hyperactivity .
	manualset3
102984	1	401467	13	NULL	NULL	NULL	NULL	Interspecies mating	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Interspecies mating triggers a RecBC-dependent SOS response in female bacteria that increases recombination mainly through overproduction of the RecA protein .
	manualset3
102985	2	401467	13	NULL	NULL	0	NULL	RecBC-dependent SOS response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interspecies mating triggers a RecBC-dependent SOS response in female bacteria that increases recombination mainly through overproduction of the RecA protein .
	manualset3
102986	3	401467	13	NULL	NULL	0	NULL	female bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Interspecies mating triggers a RecBC-dependent SOS response in female bacteria that increases recombination mainly through overproduction of the RecA protein .
	manualset3
102987	4	401467	13	NULL	NULL	0	NULL	recombination	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interspecies mating triggers a RecBC-dependent SOS response in female bacteria that increases recombination mainly through overproduction of the RecA protein .
	manualset3
102988	5	401467	13	NULL	NULL	0	NULL	overproduction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interspecies mating triggers a RecBC-dependent SOS response in female bacteria that increases recombination mainly through overproduction of the RecA protein .
	manualset3
102989	6	401467	13	NULL	NULL	0	NULL	RecA protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interspecies mating triggers a RecBC-dependent SOS response in female bacteria that increases recombination mainly through overproduction of the RecA protein .
	manualset3
102990	1	401468	13	NULL	NULL	0	NULL	Associative analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Associative analysis of the connection between mutation C1167T in the catalase gene and polymorphic marker D6S392 nearby the Mn-dependent superoxide dismutase gene with diabetic microangiopathies ) .
	manualset3
102991	2	401468	13	NULL	NULL	0	NULL	connection	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	( Associative analysis of the connection between mutation C1167T in the catalase gene and polymorphic marker D6S392 nearby the Mn-dependent superoxide dismutase gene with diabetic microangiopathies ) .
	manualset3
102992	3	401468	13	NULL	NULL	0	NULL	mutation C1167T	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Associative analysis of the connection between mutation C1167T in the catalase gene and polymorphic marker D6S392 nearby the Mn-dependent superoxide dismutase gene with diabetic microangiopathies ) .
	manualset3
102993	4	401468	13	NULL	NULL	0	NULL	catalase gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	( Associative analysis of the connection between mutation C1167T in the catalase gene and polymorphic marker D6S392 nearby the Mn-dependent superoxide dismutase gene with diabetic microangiopathies ) .
	manualset3
102994	5	401468	13	NULL	NULL	0	NULL	polymorphic marker D6S392	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	( Associative analysis of the connection between mutation C1167T in the catalase gene and polymorphic marker D6S392 nearby the Mn-dependent superoxide dismutase gene with diabetic microangiopathies ) .
	manualset3
102995	6	401468	13	NULL	NULL	0	NULL	Mn-dependent superoxide dismutase gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	( Associative analysis of the connection between mutation C1167T in the catalase gene and polymorphic marker D6S392 nearby the Mn-dependent superoxide dismutase gene with diabetic microangiopathies ) .
	manualset3
102996	7	401468	13	NULL	NULL	0	NULL	diabetic microangiopathies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Associative analysis of the connection between mutation C1167T in the catalase gene and polymorphic marker D6S392 nearby the Mn-dependent superoxide dismutase gene with diabetic microangiopathies ) .
	manualset3
102997	1	401469	13	NULL	NULL	0	NULL	3F8	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	3F8 is able to co-immunoprecipitate NS3 and NS5 from BHK-21 cells infected with DENV2 , and 3F10 is able to detect an interaction between recombinant NS2B ( CF18 ) NS3 full-length protein and the NS5 RNA-dependent RNA polymerase ( RdRp ) domain in an ELISA-based binding assay .
	manualset3
102998	2	401469	13	NULL	NULL	0	NULL	NS3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	3F8 is able to co-immunoprecipitate NS3 and NS5 from BHK-21 cells infected with DENV2 , and 3F10 is able to detect an interaction between recombinant NS2B ( CF18 ) NS3 full-length protein and the NS5 RNA-dependent RNA polymerase ( RdRp ) domain in an ELISA-based binding assay .
	manualset3
102999	3	401469	13	NULL	NULL	0	NULL	NS5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	3F8 is able to co-immunoprecipitate NS3 and NS5 from BHK-21 cells infected with DENV2 , and 3F10 is able to detect an interaction between recombinant NS2B ( CF18 ) NS3 full-length protein and the NS5 RNA-dependent RNA polymerase ( RdRp ) domain in an ELISA-based binding assay .
	manualset3
103000	4	401469	13	NULL	NULL	0	NULL	BHK-21 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	3F8 is able to co-immunoprecipitate NS3 and NS5 from BHK-21 cells infected with DENV2 , and 3F10 is able to detect an interaction between recombinant NS2B ( CF18 ) NS3 full-length protein and the NS5 RNA-dependent RNA polymerase ( RdRp ) domain in an ELISA-based binding assay .
	manualset3
103001	5	401469	13	NULL	NULL	0	NULL	DENV2	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	3F8 is able to co-immunoprecipitate NS3 and NS5 from BHK-21 cells infected with DENV2 , and 3F10 is able to detect an interaction between recombinant NS2B ( CF18 ) NS3 full-length protein and the NS5 RNA-dependent RNA polymerase ( RdRp ) domain in an ELISA-based binding assay .
	manualset3
103002	6	401469	13	NULL	NULL	0	NULL	3F10 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	3F8 is able to co-immunoprecipitate NS3 and NS5 from BHK-21 cells infected with DENV2 , and 3F10 is able to detect an interaction between recombinant NS2B ( CF18 ) NS3 full-length protein and the NS5 RNA-dependent RNA polymerase ( RdRp ) domain in an ELISA-based binding assay .
	manualset3
103003	7	401469	13	NULL	NULL	0	NULL	interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	3F8 is able to co-immunoprecipitate NS3 and NS5 from BHK-21 cells infected with DENV2 , and 3F10 is able to detect an interaction between recombinant NS2B ( CF18 ) NS3 full-length protein and the NS5 RNA-dependent RNA polymerase ( RdRp ) domain in an ELISA-based binding assay .
	manualset3
103004	8	401469	13	NULL	NULL	0	NULL	recombinant NS2B ( CF18 ) NS3 full-length protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	3F8 is able to co-immunoprecipitate NS3 and NS5 from BHK-21 cells infected with DENV2 , and 3F10 is able to detect an interaction between recombinant NS2B ( CF18 ) NS3 full-length protein and the NS5 RNA-dependent RNA polymerase ( RdRp ) domain in an ELISA-based binding assay .
	manualset3
103005	9	401469	13	NULL	NULL	0	NULL	NS5 RNA-dependent RNA polymerase ( RdRp ) domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	3F8 is able to co-immunoprecipitate NS3 and NS5 from BHK-21 cells infected with DENV2 , and 3F10 is able to detect an interaction between recombinant NS2B ( CF18 ) NS3 full-length protein and the NS5 RNA-dependent RNA polymerase ( RdRp ) domain in an ELISA-based binding assay .
	manualset3
103006	10	401469	13	NULL	NULL	0	NULL	ELISA-based binding assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	3F8 is able to co-immunoprecipitate NS3 and NS5 from BHK-21 cells infected with DENV2 , and 3F10 is able to detect an interaction between recombinant NS2B ( CF18 ) NS3 full-length protein and the NS5 RNA-dependent RNA polymerase ( RdRp ) domain in an ELISA-based binding assay .
	manualset3
103007	1	401470	13	NULL	NULL	0	NULL	Interspecies	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Interspecies transfer of female mitochondrial DNA is coupled with role-reversals and departure from neutrality in the mussel Mytilus trossulus .
	manualset3
103008	2	401470	13	NULL	NULL	0	NULL	female mitochondrial DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Interspecies transfer of female mitochondrial DNA is coupled with role-reversals and departure from neutrality in the mussel Mytilus trossulus .
	manualset3
103009	3	401470	13	NULL	NULL	0	NULL	departure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interspecies transfer of female mitochondrial DNA is coupled with role-reversals and departure from neutrality in the mussel Mytilus trossulus .
	manualset3
103010	4	401470	13	NULL	NULL	0	NULL	role-reversals 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interspecies transfer of female mitochondrial DNA is coupled with role-reversals and departure from neutrality in the mussel Mytilus trossulus .
	manualset3
103011	5	401470	13	NULL	NULL	0	NULL	neutrality	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interspecies transfer of female mitochondrial DNA is coupled with role-reversals and departure from neutrality in the mussel Mytilus trossulus .
	manualset3
103012	6	401470	13	NULL	NULL	0	NULL	mussel Mytilus trossulus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Interspecies transfer of female mitochondrial DNA is coupled with role-reversals and departure from neutrality in the mussel Mytilus trossulus .
	manualset3
103013	1	401471	13	NULL	NULL	0	NULL	Interspecies Drosophila hybrids	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Interspecies Drosophila hybrids of the virilis group were used to study the maternal effect ( expression of the recessive glossy mutation when females of D. virilis strains carrying this mutation are crossed with D. littoralis males of the wild type ) at low temperatures .
	manualset3
103014	2	401471	13	NULL	NULL	0	NULL	virilis group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Interspecies Drosophila hybrids of the virilis group were used to study the maternal effect ( expression of the recessive glossy mutation when females of D. virilis strains carrying this mutation are crossed with D. littoralis males of the wild type ) at low temperatures .
	manualset3
103015	3	401471	13	NULL	NULL	0	NULL	maternal effect 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interspecies Drosophila hybrids of the virilis group were used to study the maternal effect ( expression of the recessive glossy mutation when females of D. virilis strains carrying this mutation are crossed with D. littoralis males of the wild type ) at low temperatures .
	manualset3
103016	4	401471	13	NULL	NULL	0	NULL	expression 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interspecies Drosophila hybrids of the virilis group were used to study the maternal effect ( expression of the recessive glossy mutation when females of D. virilis strains carrying this mutation are crossed with D. littoralis males of the wild type ) at low temperatures .
	manualset3
103017	5	401471	13	NULL	NULL	0	NULL	recessive glossy mutation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interspecies Drosophila hybrids of the virilis group were used to study the maternal effect ( expression of the recessive glossy mutation when females of D. virilis strains carrying this mutation are crossed with D. littoralis males of the wild type ) at low temperatures .
	manualset3
103018	6	401471	13	NULL	NULL	0	NULL	females of D. virilis strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Interspecies Drosophila hybrids of the virilis group were used to study the maternal effect ( expression of the recessive glossy mutation when females of D. virilis strains carrying this mutation are crossed with D. littoralis males of the wild type ) at low temperatures .
	manualset3
103019	7	401471	13	NULL	NULL	0	NULL	mutation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interspecies Drosophila hybrids of the virilis group were used to study the maternal effect ( expression of the recessive glossy mutation when females of D. virilis strains carrying this mutation are crossed with D. littoralis males of the wild type ) at low temperatures .
	manualset3
103020	8	401471	13	NULL	NULL	0	NULL	D. littoralis males 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Interspecies Drosophila hybrids of the virilis group were used to study the maternal effect ( expression of the recessive glossy mutation when females of D. virilis strains carrying this mutation are crossed with D. littoralis males of the wild type ) at low temperatures .
	manualset3
103021	9	401471	13	NULL	NULL	0	NULL	low temperatures	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Interspecies Drosophila hybrids of the virilis group were used to study the maternal effect ( expression of the recessive glossy mutation when females of D. virilis strains carrying this mutation are crossed with D. littoralis males of the wild type ) at low temperatures .
	manualset3
103022	1	401472	13	NULL	NULL	0	NULL	Interspecific sequence divergence	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interspecific sequence divergence , based on mtDNA cytochrome b ( 0.118 + / - 0.01 ) , was larger than intraspecific divergences between haplotypes ( 0.007 for A. taiwanensis and 0.003 for A. berda ) .
	manualset3
103023	2	401472	13	NULL	NULL	0	NULL	mtDNA cytochrome b	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Interspecific sequence divergence , based on mtDNA cytochrome b ( 0.118 + / - 0.01 ) , was larger than intraspecific divergences between haplotypes ( 0.007 for A. taiwanensis and 0.003 for A. berda ) .
	manualset3
103024	3	401472	13	NULL	NULL	0	NULL	0.118 + / - 0.01 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Interspecific sequence divergence , based on mtDNA cytochrome b ( 0.118 + / - 0.01 ) , was larger than intraspecific divergences between haplotypes ( 0.007 for A. taiwanensis and 0.003 for A. berda ) .
	manualset3
103025	4	401472	13	NULL	NULL	0	NULL	intraspecific divergences	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interspecific sequence divergence , based on mtDNA cytochrome b ( 0.118 + / - 0.01 ) , was larger than intraspecific divergences between haplotypes ( 0.007 for A. taiwanensis and 0.003 for A. berda ) .
	manualset3
103026	5	401472	13	NULL	NULL	0	NULL	haplotypes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Interspecific sequence divergence , based on mtDNA cytochrome b ( 0.118 + / - 0.01 ) , was larger than intraspecific divergences between haplotypes ( 0.007 for A. taiwanensis and 0.003 for A. berda ) .
	manualset3
103027	6	401472	13	NULL	NULL	0	NULL	0.007	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Interspecific sequence divergence , based on mtDNA cytochrome b ( 0.118 + / - 0.01 ) , was larger than intraspecific divergences between haplotypes ( 0.007 for A. taiwanensis and 0.003 for A. berda ) .
	manualset3
103028	7	401472	13	NULL	NULL	0	NULL	A. taiwanensis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Interspecific sequence divergence , based on mtDNA cytochrome b ( 0.118 + / - 0.01 ) , was larger than intraspecific divergences between haplotypes ( 0.007 for A. taiwanensis and 0.003 for A. berda ) .
	manualset3
103029	8	401472	13	NULL	NULL	0	NULL	0.003 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Interspecific sequence divergence , based on mtDNA cytochrome b ( 0.118 + / - 0.01 ) , was larger than intraspecific divergences between haplotypes ( 0.007 for A. taiwanensis and 0.003 for A. berda ) .
	manualset3
103030	9	401472	13	NULL	NULL	0	NULL	A. berda	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Interspecific sequence divergence , based on mtDNA cytochrome b ( 0.118 + / - 0.01 ) , was larger than intraspecific divergences between haplotypes ( 0.007 for A. taiwanensis and 0.003 for A. berda ) .
	manualset3
103031	1	401473	13	NULL	NULL	0	NULL	Intervention 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Intervention following a sudden death : the social work-medical examiner model .
	manualset3
103032	2	401473	13	NULL	NULL	0	NULL	death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intervention following a sudden death : the social work-medical examiner model .
	manualset3
103033	3	401473	13	NULL	NULL	0	NULL	social work-medical examiner model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Intervention following a sudden death : the social work-medical examiner model .
	manualset3
103034	1	401474	13	NULL	NULL	0	NULL	Interventional cardiology	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Interventional cardiology : A new drug-eluting stent that does not live up to its promise .
	manualset3
103035	2	401474	13	NULL	NULL	0	NULL	drug-eluting stent	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Interventional cardiology : A new drug-eluting stent that does not live up to its promise .
	manualset3
103036	3	401474	13	NULL	NULL	0	NULL	promise	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Interventional cardiology : A new drug-eluting stent that does not live up to its promise .
	manualset3
103037	1	401475	13	NULL	NULL	0	NULL	Interventions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interventions that lower dietary ED by means of increasing fruit and vegetable intake and decreasing fat consumption may be an effective strategy for reducing childhood obesity .
	manualset3
103038	2	401475	13	NULL	NULL	0	NULL	 lower dietary ED	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Interventions that lower dietary ED by means of increasing fruit and vegetable intake and decreasing fat consumption may be an effective strategy for reducing childhood obesity .
	manualset3
103039	3	401475	13	NULL	NULL	0	NULL	fruit intake	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Interventions that lower dietary ED by means of increasing fruit and vegetable intake and decreasing fat consumption may be an effective strategy for reducing childhood obesity .
	manualset3
103040	4	401475	13	NULL	NULL	0	NULL	vegetable intake	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Interventions that lower dietary ED by means of increasing fruit and vegetable intake and decreasing fat consumption may be an effective strategy for reducing childhood obesity .
	manualset3
103041	5	401475	13	NULL	NULL	0	NULL	fat consumption	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Interventions that lower dietary ED by means of increasing fruit and vegetable intake and decreasing fat consumption may be an effective strategy for reducing childhood obesity .
	manualset3
103042	6	401475	13	NULL	NULL	0	NULL	strategy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interventions that lower dietary ED by means of increasing fruit and vegetable intake and decreasing fat consumption may be an effective strategy for reducing childhood obesity .
	manualset3
103043	7	401475	13	NULL	NULL	0	NULL	childhood obesity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Interventions that lower dietary ED by means of increasing fruit and vegetable intake and decreasing fat consumption may be an effective strategy for reducing childhood obesity .
	manualset3
103044	1	401476	13	NULL	NULL	0	NULL	3H-imipramine binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	3H-imipramine binding in platelets : influence of varying proportions of intact platelets in membrane preparations on binding .
	manualset3
103045	2	401476	13	NULL	NULL	0	NULL	platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	3H-imipramine binding in platelets : influence of varying proportions of intact platelets in membrane preparations on binding .
	manualset3
103046	3	401476	13	NULL	NULL	0	NULL	influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	3H-imipramine binding in platelets : influence of varying proportions of intact platelets in membrane preparations on binding .
	manualset3
103047	4	401476	13	NULL	NULL	0	NULL	proportions 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	3H-imipramine binding in platelets : influence of varying proportions of intact platelets in membrane preparations on binding .
	manualset3
103048	5	401476	13	NULL	NULL	0	NULL	intact platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	3H-imipramine binding in platelets : influence of varying proportions of intact platelets in membrane preparations on binding .
	manualset3
103049	6	401476	13	NULL	NULL	0	NULL	membrane preparations	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	3H-imipramine binding in platelets : influence of varying proportions of intact platelets in membrane preparations on binding .
	manualset3
103050	7	401476	13	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	3H-imipramine binding in platelets : influence of varying proportions of intact platelets in membrane preparations on binding .
	manualset3
103051	1	401477	13	NULL	NULL	0	NULL	Intestinal distribution	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intestinal distribution and leakage of hyaluronan in small bowel allografting in the rat .
	manualset3
103052	2	401477	13	NULL	NULL	0	NULL	leakage of hyaluronan	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intestinal distribution and leakage of hyaluronan in small bowel allografting in the rat .
	manualset3
103053	3	401477	13	NULL	NULL	0	NULL	small bowel allografting 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intestinal distribution and leakage of hyaluronan in small bowel allografting in the rat .
	manualset3
103054	4	401477	13	NULL	NULL	0	NULL	rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Intestinal distribution and leakage of hyaluronan in small bowel allografting in the rat .
	manualset3
103055	1	401478	13	NULL	NULL	0	NULL	Intestinal microsporidiosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intestinal microsporidiosis is recognized as an important cause of opportunistic infections in immunocompromised patients , especially those with AIDS .
	manualset3
103056	2	401478	13	NULL	NULL	0	NULL	cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intestinal microsporidiosis is recognized as an important cause of opportunistic infections in immunocompromised patients , especially those with AIDS .
	manualset3
103057	3	401478	13	NULL	NULL	0	NULL	opportunistic infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intestinal microsporidiosis is recognized as an important cause of opportunistic infections in immunocompromised patients , especially those with AIDS .
	manualset3
103058	4	401478	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Intestinal microsporidiosis is recognized as an important cause of opportunistic infections in immunocompromised patients , especially those with AIDS .
	manualset3
103059	5	401478	13	NULL	NULL	0	NULL	AIDS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Intestinal microsporidiosis is recognized as an important cause of opportunistic infections in immunocompromised patients , especially those with AIDS .
	manualset3
103060	1	401479	13	NULL	NULL	0	NULL	Intestinal trefoil factor ( TFF 3 ) mRNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Intestinal trefoil factor ( TFF 3 ) and pS2 ( TFF 1 ) , but not spasmolytic polypeptide ( TFF 2 ) mRNAs are co-expressed in normal , hyperplastic , and neoplastic human breast epithelium .
	manualset3
103061	2	401479	13	NULL	NULL	0	NULL	pS2 ( TFF 1 ) mRNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Intestinal trefoil factor ( TFF 3 ) and pS2 ( TFF 1 ) , but not spasmolytic polypeptide ( TFF 2 ) mRNAs are co-expressed in normal , hyperplastic , and neoplastic human breast epithelium .
	manualset3
103062	3	401479	13	NULL	NULL	0	NULL	spasmolytic polypeptide ( TFF 2 ) mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Intestinal trefoil factor ( TFF 3 ) and pS2 ( TFF 1 ) , but not spasmolytic polypeptide ( TFF 2 ) mRNAs are co-expressed in normal , hyperplastic , and neoplastic human breast epithelium .
	manualset3
103063	4	401479	13	NULL	NULL	0	NULL	normal human breast epithelium	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Intestinal trefoil factor ( TFF 3 ) and pS2 ( TFF 1 ) , but not spasmolytic polypeptide ( TFF 2 ) mRNAs are co-expressed in normal , hyperplastic , and neoplastic human breast epithelium .
	manualset3
103064	5	401479	13	NULL	NULL	0	NULL	hyperplastic human breast epithelium	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Intestinal trefoil factor ( TFF 3 ) and pS2 ( TFF 1 ) , but not spasmolytic polypeptide ( TFF 2 ) mRNAs are co-expressed in normal , hyperplastic , and neoplastic human breast epithelium .
	manualset3
103065	6	401479	13	NULL	NULL	0	NULL	neoplastic human breast epithelium	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Intestinal trefoil factor ( TFF 3 ) and pS2 ( TFF 1 ) , but not spasmolytic polypeptide ( TFF 2 ) mRNAs are co-expressed in normal , hyperplastic , and neoplastic human breast epithelium .
	manualset3
103066	1	401480	13	NULL	NULL	0	NULL	Intoxication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intoxication from GHB is common with GHB users .
	manualset3
103067	2	401480	13	NULL	NULL	0	NULL	GHB 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Intoxication from GHB is common with GHB users .
	manualset3
103068	3	401480	13	NULL	NULL	0	NULL	GHB users	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Intoxication from GHB is common with GHB users .
	manualset3
103178	1	401481	13	NULL	NULL	0	NULL	Intra-abdominal ligation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-abdominal ligation and transection of cryptorchid testes is an effective method for cryptorchid castration .
	manualset3
103179	2	401481	13	NULL	NULL	0	NULL	 transection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-abdominal ligation and transection of cryptorchid testes is an effective method for cryptorchid castration .
	manualset3
103180	3	401481	13	NULL	NULL	0	NULL	cryptorchid testes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-abdominal ligation and transection of cryptorchid testes is an effective method for cryptorchid castration .
	manualset3
103181	4	401481	13	NULL	NULL	0	NULL	effective method 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-abdominal ligation and transection of cryptorchid testes is an effective method for cryptorchid castration .
	manualset3
103182	5	401481	13	NULL	NULL	0	NULL	cryptorchid castration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-abdominal ligation and transection of cryptorchid testes is an effective method for cryptorchid castration .
	manualset3
103183	1	401482	13	NULL	NULL	0	NULL	3a	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	3a forms a strong 1 : 1 complex with paraquat ( 1 ) in acetone solution with a high apparent association constant , 1.4 x 10 ( 4 ) M ( - ) ( 1 ) .
	manualset3
103184	2	401482	13	NULL	NULL	0	NULL	1 : 1 complex	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	3a forms a strong 1 : 1 complex with paraquat ( 1 ) in acetone solution with a high apparent association constant , 1.4 x 10 ( 4 ) M ( - ) ( 1 ) .
	manualset3
103185	3	401482	13	NULL	NULL	0	NULL	paraquat ( 1 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	3a forms a strong 1 : 1 complex with paraquat ( 1 ) in acetone solution with a high apparent association constant , 1.4 x 10 ( 4 ) M ( - ) ( 1 ) .
	manualset3
103186	4	401482	13	NULL	NULL	0	NULL	acetone solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	3a forms a strong 1 : 1 complex with paraquat ( 1 ) in acetone solution with a high apparent association constant , 1.4 x 10 ( 4 ) M ( - ) ( 1 ) .
	manualset3
103187	5	401482	13	NULL	NULL	0	NULL	association constant 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	3a forms a strong 1 : 1 complex with paraquat ( 1 ) in acetone solution with a high apparent association constant , 1.4 x 10 ( 4 ) M ( - ) ( 1 ) .
	manualset3
103188	6	401482	13	NULL	NULL	0	NULL	1.4 x 10 ( 4 ) M ( - ) ( 1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	3a forms a strong 1 : 1 complex with paraquat ( 1 ) in acetone solution with a high apparent association constant , 1.4 x 10 ( 4 ) M ( - ) ( 1 ) .
	manualset3
103189	1	401483	13	NULL	NULL	0	NULL	Intra-arterial administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-arterial administration of glucagon ( 10-100 mug ) into the perfused pancreas also elicited increased secretion .
	manualset3
103190	2	401483	13	NULL	NULL	0	NULL	glucagon	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-arterial administration of glucagon ( 10-100 mug ) into the perfused pancreas also elicited increased secretion .
	manualset3
103191	3	401483	13	NULL	NULL	0	NULL	10-100 mug	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-arterial administration of glucagon ( 10-100 mug ) into the perfused pancreas also elicited increased secretion .
	manualset3
103192	4	401483	13	NULL	NULL	0	NULL	pancreas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-arterial administration of glucagon ( 10-100 mug ) into the perfused pancreas also elicited increased secretion .
	manualset3
103193	5	401483	13	NULL	NULL	0	NULL	secretion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-arterial administration of glucagon ( 10-100 mug ) into the perfused pancreas also elicited increased secretion .
	manualset3
103194	1	401484	13	NULL	NULL	NULL	NULL	Intra-assay coefficients of variation 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Intra-assay coefficients of variation ranged from 3.1 % to 4.2 % in the 10-40 fmol/well concentration range , and interassay coefficients of variation ranged from 3.5 % to 4.5 % in the 550-950 fmol/ml range .
	manualset3
103195	2	401484	13	NULL	NULL	0	NULL	3.1 % to 4.2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-assay coefficients of variation ranged from 3.1 % to 4.2 % in the 10-40 fmol/well concentration range , and interassay coefficients of variation ranged from 3.5 % to 4.5 % in the 550-950 fmol/ml range .
	manualset3
103196	3	401484	13	NULL	NULL	0	NULL	10-40 fmol/well concentration range	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-assay coefficients of variation ranged from 3.1 % to 4.2 % in the 10-40 fmol/well concentration range , and interassay coefficients of variation ranged from 3.5 % to 4.5 % in the 550-950 fmol/ml range .
	manualset3
103197	4	401484	13	NULL	NULL	0	NULL	interassay coefficients of variation	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-assay coefficients of variation ranged from 3.1 % to 4.2 % in the 10-40 fmol/well concentration range , and interassay coefficients of variation ranged from 3.5 % to 4.5 % in the 550-950 fmol/ml range .
	manualset3
103198	5	401484	13	NULL	NULL	0	NULL	3.5 % to 4.5 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-assay coefficients of variation ranged from 3.1 % to 4.2 % in the 10-40 fmol/well concentration range , and interassay coefficients of variation ranged from 3.5 % to 4.5 % in the 550-950 fmol/ml range .
	manualset3
103199	6	401484	13	NULL	NULL	0	NULL	550-950 fmol/ml range	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-assay coefficients of variation ranged from 3.1 % to 4.2 % in the 10-40 fmol/well concentration range , and interassay coefficients of variation ranged from 3.5 % to 4.5 % in the 550-950 fmol/ml range .
	manualset3
103200	1	401485	13	NULL	NULL	0	NULL	Intra-operative findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-operative findings in varus osteoarthritis of the knee .
	manualset3
103201	2	401485	13	NULL	NULL	0	NULL	varus osteoarthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-operative findings in varus osteoarthritis of the knee .
	manualset3
103202	3	401485	13	NULL	NULL	0	NULL	knee	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-operative findings in varus osteoarthritis of the knee .
	manualset3
103203	1	401486	13	NULL	NULL	0	NULL	Intra-pair differences	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-pair differences between patients and their non-ill co-twins in hippocampal volume and memory performance were highly positively correlated .
	manualset3
103204	2	401486	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-pair differences between patients and their non-ill co-twins in hippocampal volume and memory performance were highly positively correlated .
	manualset3
103205	3	401486	13	NULL	NULL	0	NULL	non-ill co-twins	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-pair differences between patients and their non-ill co-twins in hippocampal volume and memory performance were highly positively correlated .
	manualset3
103206	4	401486	13	NULL	NULL	0	NULL	hippocampal volume	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-pair differences between patients and their non-ill co-twins in hippocampal volume and memory performance were highly positively correlated .
	manualset3
103207	5	401486	13	NULL	NULL	0	NULL	memory performance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-pair differences between patients and their non-ill co-twins in hippocampal volume and memory performance were highly positively correlated .
	manualset3
103208	1	401487	13	NULL	NULL	0	NULL	Intracage ammonia levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracage ammonia levels , bacterial growth , and absorptive capacity of bedding were measured for cages of C57BL/6 mice under nonautoclaved and autoclaved conditions on static and ventilated racks in a barrier facility .
	manualset3
103209	2	401487	13	NULL	NULL	0	NULL	bacterial growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracage ammonia levels , bacterial growth , and absorptive capacity of bedding were measured for cages of C57BL/6 mice under nonautoclaved and autoclaved conditions on static and ventilated racks in a barrier facility .
	manualset3
103210	3	401487	13	NULL	NULL	0	NULL	absorptive capacity 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracage ammonia levels , bacterial growth , and absorptive capacity of bedding were measured for cages of C57BL/6 mice under nonautoclaved and autoclaved conditions on static and ventilated racks in a barrier facility .
	manualset3
103211	4	401487	13	NULL	NULL	0	NULL	bedding 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracage ammonia levels , bacterial growth , and absorptive capacity of bedding were measured for cages of C57BL/6 mice under nonautoclaved and autoclaved conditions on static and ventilated racks in a barrier facility .
	manualset3
103212	5	401487	13	NULL	NULL	0	NULL	cages 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracage ammonia levels , bacterial growth , and absorptive capacity of bedding were measured for cages of C57BL/6 mice under nonautoclaved and autoclaved conditions on static and ventilated racks in a barrier facility .
	manualset3
103213	6	401487	13	NULL	NULL	0	NULL	C57BL/6 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracage ammonia levels , bacterial growth , and absorptive capacity of bedding were measured for cages of C57BL/6 mice under nonautoclaved and autoclaved conditions on static and ventilated racks in a barrier facility .
	manualset3
103214	7	401487	13	NULL	NULL	0	NULL	nonautoclaved conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracage ammonia levels , bacterial growth , and absorptive capacity of bedding were measured for cages of C57BL/6 mice under nonautoclaved and autoclaved conditions on static and ventilated racks in a barrier facility .
	manualset3
103215	8	401487	13	NULL	NULL	0	NULL	autoclaved conditions 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracage ammonia levels , bacterial growth , and absorptive capacity of bedding were measured for cages of C57BL/6 mice under nonautoclaved and autoclaved conditions on static and ventilated racks in a barrier facility .
	manualset3
103216	9	401487	13	NULL	NULL	0	NULL	racks	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracage ammonia levels , bacterial growth , and absorptive capacity of bedding were measured for cages of C57BL/6 mice under nonautoclaved and autoclaved conditions on static and ventilated racks in a barrier facility .
	manualset3
103217	10	401487	13	NULL	NULL	0	NULL	barrier facility	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracage ammonia levels , bacterial growth , and absorptive capacity of bedding were measured for cages of C57BL/6 mice under nonautoclaved and autoclaved conditions on static and ventilated racks in a barrier facility .
	manualset3
103383	1	401488	13	NULL	NULL	0	NULL	Intracellular Ca ( 2 + ) 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular Ca ( 2 + ) remains fairly constant under all these conditions .
	manualset3
103384	2	401488	13	NULL	NULL	0	NULL	conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular Ca ( 2 + ) remains fairly constant under all these conditions .
	manualset3
103385	1	401489	13	NULL	NULL	0	NULL	Intracellular Ca2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular Ca2 + concentration in the N1E-115 neuronal cell line and its use for peripheric nerve regeneration .
	manualset3
103386	2	401489	13	NULL	NULL	0	NULL	concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular Ca2 + concentration in the N1E-115 neuronal cell line and its use for peripheric nerve regeneration .
	manualset3
103387	3	401489	13	NULL	NULL	0	NULL	N1E-115 neuronal cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular Ca2 + concentration in the N1E-115 neuronal cell line and its use for peripheric nerve regeneration .
	manualset3
103388	4	401489	13	NULL	NULL	0	NULL	peripheric nerve regeneration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular Ca2 + concentration in the N1E-115 neuronal cell line and its use for peripheric nerve regeneration .
	manualset3
103389	5	401489	13	NULL	NULL	0	NULL	use	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular Ca2 + concentration in the N1E-115 neuronal cell line and its use for peripheric nerve regeneration .
	manualset3
103390	1	401490	13	NULL	NULL	0	NULL	4-MC-administered ACR neuropathy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	4-MC-administered ACR neuropathy rats showed improvement , i.e. , a decrease in landing foot spread distance , increase in motor nerve conduction velocity and increase in nerve growth factor content in the sciatic nerves in comparison with the corresponding values for ACR neuropathy rats given phosphate-buffered saline alone .
	manualset3
103391	2	401490	13	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	4-MC-administered ACR neuropathy rats showed improvement , i.e. , a decrease in landing foot spread distance , increase in motor nerve conduction velocity and increase in nerve growth factor content in the sciatic nerves in comparison with the corresponding values for ACR neuropathy rats given phosphate-buffered saline alone .
	manualset3
103392	3	401490	13	NULL	NULL	0	NULL	improvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	4-MC-administered ACR neuropathy rats showed improvement , i.e. , a decrease in landing foot spread distance , increase in motor nerve conduction velocity and increase in nerve growth factor content in the sciatic nerves in comparison with the corresponding values for ACR neuropathy rats given phosphate-buffered saline alone .
	manualset3
103393	4	401490	13	NULL	NULL	0	NULL	landing foot spread distance	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	4-MC-administered ACR neuropathy rats showed improvement , i.e. , a decrease in landing foot spread distance , increase in motor nerve conduction velocity and increase in nerve growth factor content in the sciatic nerves in comparison with the corresponding values for ACR neuropathy rats given phosphate-buffered saline alone .
	manualset3
103394	5	401490	13	NULL	NULL	0	NULL	decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	4-MC-administered ACR neuropathy rats showed improvement , i.e. , a decrease in landing foot spread distance , increase in motor nerve conduction velocity and increase in nerve growth factor content in the sciatic nerves in comparison with the corresponding values for ACR neuropathy rats given phosphate-buffered saline alone .
	manualset3
103395	6	401490	13	NULL	NULL	0	NULL	 increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	4-MC-administered ACR neuropathy rats showed improvement , i.e. , a decrease in landing foot spread distance , increase in motor nerve conduction velocity and increase in nerve growth factor content in the sciatic nerves in comparison with the corresponding values for ACR neuropathy rats given phosphate-buffered saline alone .
	manualset3
103396	7	401490	13	NULL	NULL	0	NULL	 motor nerve conduction velocity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	4-MC-administered ACR neuropathy rats showed improvement , i.e. , a decrease in landing foot spread distance , increase in motor nerve conduction velocity and increase in nerve growth factor content in the sciatic nerves in comparison with the corresponding values for ACR neuropathy rats given phosphate-buffered saline alone .
	manualset3
103397	8	401490	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	4-MC-administered ACR neuropathy rats showed improvement , i.e. , a decrease in landing foot spread distance , increase in motor nerve conduction velocity and increase in nerve growth factor content in the sciatic nerves in comparison with the corresponding values for ACR neuropathy rats given phosphate-buffered saline alone .
	manualset3
103398	9	401490	13	NULL	NULL	0	NULL	nerve growth factor content 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	4-MC-administered ACR neuropathy rats showed improvement , i.e. , a decrease in landing foot spread distance , increase in motor nerve conduction velocity and increase in nerve growth factor content in the sciatic nerves in comparison with the corresponding values for ACR neuropathy rats given phosphate-buffered saline alone .
	manualset3
103399	10	401490	13	NULL	NULL	0	NULL	sciatic nerves	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	4-MC-administered ACR neuropathy rats showed improvement , i.e. , a decrease in landing foot spread distance , increase in motor nerve conduction velocity and increase in nerve growth factor content in the sciatic nerves in comparison with the corresponding values for ACR neuropathy rats given phosphate-buffered saline alone .
	manualset3
103400	11	401490	13	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	4-MC-administered ACR neuropathy rats showed improvement , i.e. , a decrease in landing foot spread distance , increase in motor nerve conduction velocity and increase in nerve growth factor content in the sciatic nerves in comparison with the corresponding values for ACR neuropathy rats given phosphate-buffered saline alone .
	manualset3
103401	12	401490	13	NULL	NULL	0	NULL	values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	4-MC-administered ACR neuropathy rats showed improvement , i.e. , a decrease in landing foot spread distance , increase in motor nerve conduction velocity and increase in nerve growth factor content in the sciatic nerves in comparison with the corresponding values for ACR neuropathy rats given phosphate-buffered saline alone .
	manualset3
103402	13	401490	13	NULL	NULL	0	NULL	ACR neuropathy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	4-MC-administered ACR neuropathy rats showed improvement , i.e. , a decrease in landing foot spread distance , increase in motor nerve conduction velocity and increase in nerve growth factor content in the sciatic nerves in comparison with the corresponding values for ACR neuropathy rats given phosphate-buffered saline alone .
	manualset3
103403	14	401490	13	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	4-MC-administered ACR neuropathy rats showed improvement , i.e. , a decrease in landing foot spread distance , increase in motor nerve conduction velocity and increase in nerve growth factor content in the sciatic nerves in comparison with the corresponding values for ACR neuropathy rats given phosphate-buffered saline alone .
	manualset3
103404	15	401490	13	NULL	NULL	0	NULL	phosphate-buffered saline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	4-MC-administered ACR neuropathy rats showed improvement , i.e. , a decrease in landing foot spread distance , increase in motor nerve conduction velocity and increase in nerve growth factor content in the sciatic nerves in comparison with the corresponding values for ACR neuropathy rats given phosphate-buffered saline alone .
	manualset3
103405	1	401491	13	NULL	NULL	0	NULL	Intracellular K	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular K and the Na , K and Cl permeability ratios and electrogenic Na pump activity were assessed electrophysiologically in normotension and hypertension .
	manualset3
103406	2	401491	13	NULL	NULL	0	NULL	Na permeability ratio	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular K and the Na , K and Cl permeability ratios and electrogenic Na pump activity were assessed electrophysiologically in normotension and hypertension .
	manualset3
103407	3	401491	13	NULL	NULL	0	NULL	K permeability ratio	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular K and the Na , K and Cl permeability ratios and electrogenic Na pump activity were assessed electrophysiologically in normotension and hypertension .
	manualset3
103408	4	401491	13	NULL	NULL	0	NULL	Cl permeability ratio	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular K and the Na , K and Cl permeability ratios and electrogenic Na pump activity were assessed electrophysiologically in normotension and hypertension .
	manualset3
103409	5	401491	13	NULL	NULL	0	NULL	electrogenic Na pump activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular K and the Na , K and Cl permeability ratios and electrogenic Na pump activity were assessed electrophysiologically in normotension and hypertension .
	manualset3
103410	6	401491	13	NULL	NULL	0	NULL	normotension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular K and the Na , K and Cl permeability ratios and electrogenic Na pump activity were assessed electrophysiologically in normotension and hypertension .
	manualset3
103411	7	401491	13	NULL	NULL	0	NULL	 hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular K and the Na , K and Cl permeability ratios and electrogenic Na pump activity were assessed electrophysiologically in normotension and hypertension .
	manualset3
103412	1	401492	13	NULL	NULL	0	NULL	Intracellular NEP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular NEP developed HNE adducts after 24 hours of HNE or Abeta treatment as determined by immunoprecipitation , immunoblotting , and double immunofluorescence staining .
	manualset3
103413	2	401492	13	NULL	NULL	0	NULL	HNE adducts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular NEP developed HNE adducts after 24 hours of HNE or Abeta treatment as determined by immunoprecipitation , immunoblotting , and double immunofluorescence staining .
	manualset3
103414	3	401492	13	NULL	NULL	0	NULL	24 hours 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular NEP developed HNE adducts after 24 hours of HNE or Abeta treatment as determined by immunoprecipitation , immunoblotting , and double immunofluorescence staining .
	manualset3
103415	4	401492	13	NULL	NULL	0	NULL	HNE	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular NEP developed HNE adducts after 24 hours of HNE or Abeta treatment as determined by immunoprecipitation , immunoblotting , and double immunofluorescence staining .
	manualset3
103416	5	401492	13	NULL	NULL	0	NULL	Abeta	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular NEP developed HNE adducts after 24 hours of HNE or Abeta treatment as determined by immunoprecipitation , immunoblotting , and double immunofluorescence staining .
	manualset3
103417	6	401492	13	NULL	NULL	0	NULL	treatment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular NEP developed HNE adducts after 24 hours of HNE or Abeta treatment as determined by immunoprecipitation , immunoblotting , and double immunofluorescence staining .
	manualset3
103418	7	401492	13	NULL	NULL	0	NULL	immunoprecipitation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular NEP developed HNE adducts after 24 hours of HNE or Abeta treatment as determined by immunoprecipitation , immunoblotting , and double immunofluorescence staining .
	manualset3
103419	8	401492	13	NULL	NULL	0	NULL	immunoblotting 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular NEP developed HNE adducts after 24 hours of HNE or Abeta treatment as determined by immunoprecipitation , immunoblotting , and double immunofluorescence staining .
	manualset3
103420	9	401492	13	NULL	NULL	0	NULL	double immunofluorescence staining 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular NEP developed HNE adducts after 24 hours of HNE or Abeta treatment as determined by immunoprecipitation , immunoblotting , and double immunofluorescence staining .
	manualset3
103421	1	401493	13	NULL	NULL	0	NULL	Intracellular accumulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular accumulation of D-xylose occurs in diaphragm of insulin-treated rats at plasma concentrations of D-xylose ranging from 4 to 2200 microg/ml ; however , a `` saturation '' phenomenon appears to be operative , since intracellular distribution declines as plasma D-xylose concentration is increased within this range .
	manualset3
103422	2	401493	13	NULL	NULL	0	NULL	 D-xylose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular accumulation of D-xylose occurs in diaphragm of insulin-treated rats at plasma concentrations of D-xylose ranging from 4 to 2200 microg/ml ; however , a `` saturation '' phenomenon appears to be operative , since intracellular distribution declines as plasma D-xylose concentration is increased within this range .
	manualset3
103423	3	401493	13	NULL	NULL	0	NULL	diaphragm	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular accumulation of D-xylose occurs in diaphragm of insulin-treated rats at plasma concentrations of D-xylose ranging from 4 to 2200 microg/ml ; however , a `` saturation '' phenomenon appears to be operative , since intracellular distribution declines as plasma D-xylose concentration is increased within this range .
	manualset3
103424	4	401493	13	NULL	NULL	0	NULL	insulin-treated rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular accumulation of D-xylose occurs in diaphragm of insulin-treated rats at plasma concentrations of D-xylose ranging from 4 to 2200 microg/ml ; however , a `` saturation '' phenomenon appears to be operative , since intracellular distribution declines as plasma D-xylose concentration is increased within this range .
	manualset3
103425	5	401493	13	NULL	NULL	0	NULL	 plasma concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular accumulation of D-xylose occurs in diaphragm of insulin-treated rats at plasma concentrations of D-xylose ranging from 4 to 2200 microg/ml ; however , a `` saturation '' phenomenon appears to be operative , since intracellular distribution declines as plasma D-xylose concentration is increased within this range .
	manualset3
103426	6	401493	13	NULL	NULL	0	NULL	D-xylose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular accumulation of D-xylose occurs in diaphragm of insulin-treated rats at plasma concentrations of D-xylose ranging from 4 to 2200 microg/ml ; however , a `` saturation '' phenomenon appears to be operative , since intracellular distribution declines as plasma D-xylose concentration is increased within this range .
	manualset3
103427	7	401493	13	NULL	NULL	0	NULL	4 to 2200 microg/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular accumulation of D-xylose occurs in diaphragm of insulin-treated rats at plasma concentrations of D-xylose ranging from 4 to 2200 microg/ml ; however , a `` saturation '' phenomenon appears to be operative , since intracellular distribution declines as plasma D-xylose concentration is increased within this range .
	manualset3
103428	8	401493	13	NULL	NULL	0	NULL	`` saturation '' 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular accumulation of D-xylose occurs in diaphragm of insulin-treated rats at plasma concentrations of D-xylose ranging from 4 to 2200 microg/ml ; however , a `` saturation '' phenomenon appears to be operative , since intracellular distribution declines as plasma D-xylose concentration is increased within this range .
	manualset3
103429	9	401493	13	NULL	NULL	0	NULL	phenomenon	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular accumulation of D-xylose occurs in diaphragm of insulin-treated rats at plasma concentrations of D-xylose ranging from 4 to 2200 microg/ml ; however , a `` saturation '' phenomenon appears to be operative , since intracellular distribution declines as plasma D-xylose concentration is increased within this range .
	manualset3
103430	10	401493	13	NULL	NULL	0	NULL	intracellular distribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular accumulation of D-xylose occurs in diaphragm of insulin-treated rats at plasma concentrations of D-xylose ranging from 4 to 2200 microg/ml ; however , a `` saturation '' phenomenon appears to be operative , since intracellular distribution declines as plasma D-xylose concentration is increased within this range .
	manualset3
103431	11	401493	13	NULL	NULL	0	NULL	plasma D-xylose concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular accumulation of D-xylose occurs in diaphragm of insulin-treated rats at plasma concentrations of D-xylose ranging from 4 to 2200 microg/ml ; however , a `` saturation '' phenomenon appears to be operative , since intracellular distribution declines as plasma D-xylose concentration is increased within this range .
	manualset3
103432	12	401493	13	NULL	NULL	0	NULL	range	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular accumulation of D-xylose occurs in diaphragm of insulin-treated rats at plasma concentrations of D-xylose ranging from 4 to 2200 microg/ml ; however , a `` saturation '' phenomenon appears to be operative , since intracellular distribution declines as plasma D-xylose concentration is increased within this range .
	manualset3
103433	1	401494	13	NULL	NULL	NULL	NULL	human CD8 ( + ) cytotoxic T lymphocyte-mediated xenocytotoxicity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Intracellular and extracellular remodeling effectively prevents human CD8 ( + ) cytotoxic T lymphocyte-mediated xenocytotoxicity by coexpression of membrane-bound human FasL and pig c-FLIP ( L ) in pig endothelial cells .
	manualset3
103434	2	401494	13	NULL	NULL	NULL	NULL	coexpression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Intracellular and extracellular remodeling effectively prevents human CD8 ( + ) cytotoxic T lymphocyte-mediated xenocytotoxicity by coexpression of membrane-bound human FasL and pig c-FLIP ( L ) in pig endothelial cells .
	manualset3
103435	3	401494	13	NULL	NULL	0	NULL	membrane-bound human FasL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular and extracellular remodeling effectively prevents human CD8 ( + ) cytotoxic T lymphocyte-mediated xenocytotoxicity by coexpression of membrane-bound human FasL and pig c-FLIP ( L ) in pig endothelial cells .
	manualset3
103436	4	401494	13	NULL	NULL	0	NULL	pig c-FLIP ( L )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular and extracellular remodeling effectively prevents human CD8 ( + ) cytotoxic T lymphocyte-mediated xenocytotoxicity by coexpression of membrane-bound human FasL and pig c-FLIP ( L ) in pig endothelial cells .
	manualset3
103437	5	401494	13	NULL	NULL	0	NULL	pig endothelial cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular and extracellular remodeling effectively prevents human CD8 ( + ) cytotoxic T lymphocyte-mediated xenocytotoxicity by coexpression of membrane-bound human FasL and pig c-FLIP ( L ) in pig endothelial cells .
	manualset3
103438	1	401495	13	NULL	NULL	NULL	NULL	Intracellular cholesterol changes 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Intracellular cholesterol changes induced by translocator protein ( 18 kDa ) TSPO/PBR ligands .
	manualset3
103439	2	401495	13	NULL	NULL	NULL	NULL	translocator protein ( 18 kDa ) TSPO/PBR ligands	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Intracellular cholesterol changes induced by translocator protein ( 18 kDa ) TSPO/PBR ligands .
	manualset3
103440	1	401496	13	NULL	NULL	0	NULL	Intracellular injection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular injection of TEA or external application of aminopyridine or apamine had little or no effect on the TEA-resistant slow tail current .
	manualset3
103441	2	401496	13	NULL	NULL	0	NULL	TEA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular injection of TEA or external application of aminopyridine or apamine had little or no effect on the TEA-resistant slow tail current .
	manualset3
103442	3	401496	13	NULL	NULL	0	NULL	external application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular injection of TEA or external application of aminopyridine or apamine had little or no effect on the TEA-resistant slow tail current .
	manualset3
103443	4	401496	13	NULL	NULL	0	NULL	aminopyridine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular injection of TEA or external application of aminopyridine or apamine had little or no effect on the TEA-resistant slow tail current .
	manualset3
103444	5	401496	13	NULL	NULL	0	NULL	apamine	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular injection of TEA or external application of aminopyridine or apamine had little or no effect on the TEA-resistant slow tail current .
	manualset3
103445	6	401496	13	NULL	NULL	0	NULL	effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular injection of TEA or external application of aminopyridine or apamine had little or no effect on the TEA-resistant slow tail current .
	manualset3
103446	7	401496	13	NULL	NULL	0	NULL	TEA-resistant slow tail current	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular injection of TEA or external application of aminopyridine or apamine had little or no effect on the TEA-resistant slow tail current .
	manualset3
103447	1	401497	13	NULL	NULL	0	NULL	Intracellular potassium concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular potassium concentrations were similar in all age groups ( 163 to 167 mEq/liter ) .
	manualset3
103448	2	401497	13	NULL	NULL	0	NULL	age groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular potassium concentrations were similar in all age groups ( 163 to 167 mEq/liter ) .
	manualset3
103449	3	401497	13	NULL	NULL	0	NULL	163 to 167 mEq/liter 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular potassium concentrations were similar in all age groups ( 163 to 167 mEq/liter ) .
	manualset3
103450	1	401498	13	NULL	NULL	0	NULL	Intracellular signaling pathways 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular signaling pathways involved in the survival of proliferating L1210 leukemia cells were investigated by using specific modulators .
	manualset3
103451	2	401498	13	NULL	NULL	0	NULL	 survival 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular signaling pathways involved in the survival of proliferating L1210 leukemia cells were investigated by using specific modulators .
	manualset3
103452	3	401498	13	NULL	NULL	0	NULL	proliferating L1210 leukemia cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular signaling pathways involved in the survival of proliferating L1210 leukemia cells were investigated by using specific modulators .
	manualset3
103453	4	401498	13	NULL	NULL	0	NULL	modulators	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular signaling pathways involved in the survival of proliferating L1210 leukemia cells were investigated by using specific modulators .
	manualset3
103454	1	401499	13	NULL	NULL	0	NULL	4-OT 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	4-OT is a member of the tautomerase superfamily , a group of homologous proteins that are characterized by a -- structural fold and a catalytic amino-terminal proline .
	manualset3
103455	2	401499	13	NULL	NULL	0	NULL	member of the tautomerase superfamily	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	4-OT is a member of the tautomerase superfamily , a group of homologous proteins that are characterized by a -- structural fold and a catalytic amino-terminal proline .
	manualset3
103456	3	401499	13	NULL	NULL	0	NULL	a group of homologous proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	4-OT is a member of the tautomerase superfamily , a group of homologous proteins that are characterized by a -- structural fold and a catalytic amino-terminal proline .
	manualset3
103457	4	401499	13	NULL	NULL	0	NULL	structural fold	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	4-OT is a member of the tautomerase superfamily , a group of homologous proteins that are characterized by a -- structural fold and a catalytic amino-terminal proline .
	manualset3
103458	5	401499	13	NULL	NULL	0	NULL	 catalytic amino-terminal proline 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	4-OT is a member of the tautomerase superfamily , a group of homologous proteins that are characterized by a -- structural fold and a catalytic amino-terminal proline .
	manualset3
103459	1	401500	13	NULL	NULL	0	NULL	Intracoronal isolating barriers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracoronal isolating barriers : effect of location on root leakage and effectiveness of bleaching agents .
	manualset3
103460	2	401500	13	NULL	NULL	0	NULL	effect of location	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracoronal isolating barriers : effect of location on root leakage and effectiveness of bleaching agents .
	manualset3
103461	3	401500	13	NULL	NULL	0	NULL	root leakage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracoronal isolating barriers : effect of location on root leakage and effectiveness of bleaching agents .
	manualset3
103462	4	401500	13	NULL	NULL	0	NULL	effectiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracoronal isolating barriers : effect of location on root leakage and effectiveness of bleaching agents .
	manualset3
103463	5	401500	13	NULL	NULL	0	NULL	bleaching agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracoronal isolating barriers : effect of location on root leakage and effectiveness of bleaching agents .
	manualset3
103464	1	401501	13	NULL	NULL	0	NULL	Intracoronary adenosine	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracoronary adenosine ( 100 ng/kg ) increased CBF by 12.4 + / - 1.4 ml .
	manualset3
103465	2	401501	13	NULL	NULL	0	NULL	100 ng/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracoronary adenosine ( 100 ng/kg ) increased CBF by 12.4 + / - 1.4 ml .
	manualset3
103466	3	401501	13	NULL	NULL	0	NULL	CBF	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracoronary adenosine ( 100 ng/kg ) increased CBF by 12.4 + / - 1.4 ml .
	manualset3
103467	4	401501	13	NULL	NULL	0	NULL	12.4 + / - 1.4 ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracoronary adenosine ( 100 ng/kg ) increased CBF by 12.4 + / - 1.4 ml .
	manualset3
103468	1	401502	13	NULL	NULL	0	NULL	Intracoronary administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracoronary administration of autologous mesenchymal stem cells in a critically ill patient with dilated cardiomyopathy .
	manualset3
103469	2	401502	13	NULL	NULL	0	NULL	 autologous mesenchymal stem cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracoronary administration of autologous mesenchymal stem cells in a critically ill patient with dilated cardiomyopathy .
	manualset3
103470	3	401502	13	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracoronary administration of autologous mesenchymal stem cells in a critically ill patient with dilated cardiomyopathy .
	manualset3
103471	4	401502	13	NULL	NULL	0	NULL	dilated cardiomyopathy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracoronary administration of autologous mesenchymal stem cells in a critically ill patient with dilated cardiomyopathy .
	manualset3
103472	1	401503	13	NULL	NULL	0	NULL	Intracoronary delivery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracoronary delivery of umbilical cord blood derived unrestricted somatic stem cells is not suitable to improve LV function after myocardial infarction in swine .
	manualset3
103473	2	401503	13	NULL	NULL	0	NULL	umbilical cord blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracoronary delivery of umbilical cord blood derived unrestricted somatic stem cells is not suitable to improve LV function after myocardial infarction in swine .
	manualset3
103474	3	401503	13	NULL	NULL	0	NULL	somatic stem cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracoronary delivery of umbilical cord blood derived unrestricted somatic stem cells is not suitable to improve LV function after myocardial infarction in swine .
	manualset3
103475	4	401503	13	NULL	NULL	0	NULL	LV function 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracoronary delivery of umbilical cord blood derived unrestricted somatic stem cells is not suitable to improve LV function after myocardial infarction in swine .
	manualset3
103476	5	401503	13	NULL	NULL	0	NULL	myocardial infarction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracoronary delivery of umbilical cord blood derived unrestricted somatic stem cells is not suitable to improve LV function after myocardial infarction in swine .
	manualset3
103477	6	401503	13	NULL	NULL	0	NULL	swine	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracoronary delivery of umbilical cord blood derived unrestricted somatic stem cells is not suitable to improve LV function after myocardial infarction in swine .
	manualset3
103478	1	401504	13	NULL	NULL	0	NULL	Intractable complex partial seizure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intractable complex partial seizure : correlation of magnetic resonance imaging with pathology and electroencephalography .
	manualset3
103479	2	401504	13	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Intractable complex partial seizure : correlation of magnetic resonance imaging with pathology and electroencephalography .
	manualset3
103480	3	401504	13	NULL	NULL	0	NULL	magnetic resonance imaging 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intractable complex partial seizure : correlation of magnetic resonance imaging with pathology and electroencephalography .
	manualset3
103481	4	401504	13	NULL	NULL	0	NULL	pathology 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intractable complex partial seizure : correlation of magnetic resonance imaging with pathology and electroencephalography .
	manualset3
103482	5	401504	13	NULL	NULL	0	NULL	electroencephalography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intractable complex partial seizure : correlation of magnetic resonance imaging with pathology and electroencephalography .
	manualset3
103483	1	401505	13	NULL	NULL	0	NULL	Intradermal blue dye	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Intradermal blue dye to identify sentinel lymph-node in breast cancer .
	manualset3
103484	2	401505	13	NULL	NULL	0	NULL	sentinel lymph-node	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Intradermal blue dye to identify sentinel lymph-node in breast cancer .
	manualset3
103485	3	401505	13	NULL	NULL	0	NULL	breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Intradermal blue dye to identify sentinel lymph-node in breast cancer .
	manualset3
103486	1	401506	13	NULL	NULL	0	NULL	Intraduodenal lipids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraduodenal lipids also stimulated circulating levels of gastrin and vasoactive intestinal polypeptide .
	manualset3
103487	2	401506	13	NULL	NULL	NULL	NULL	circulating levels 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Intraduodenal lipids also stimulated circulating levels of gastrin and vasoactive intestinal polypeptide .
	manualset3
103488	3	401506	13	NULL	NULL	0	NULL	gastrin 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraduodenal lipids also stimulated circulating levels of gastrin and vasoactive intestinal polypeptide .
	manualset3
103489	4	401506	13	NULL	NULL	0	NULL	vasoactive intestinal polypeptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraduodenal lipids also stimulated circulating levels of gastrin and vasoactive intestinal polypeptide .
	manualset3
103490	1	401507	13	NULL	NULL	0	NULL	Intramuscular pressure 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intramuscular pressure was higher during isometric contraction than during eccentric and concentric activity , and the torque was in between the two latter contraction modes .
	manualset3
103491	2	401507	13	NULL	NULL	0	NULL	isometric contraction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intramuscular pressure was higher during isometric contraction than during eccentric and concentric activity , and the torque was in between the two latter contraction modes .
	manualset3
103492	3	401507	13	NULL	NULL	0	NULL	eccentric activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intramuscular pressure was higher during isometric contraction than during eccentric and concentric activity , and the torque was in between the two latter contraction modes .
	manualset3
103493	4	401507	13	NULL	NULL	0	NULL	concentric activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intramuscular pressure was higher during isometric contraction than during eccentric and concentric activity , and the torque was in between the two latter contraction modes .
	manualset3
103494	5	401507	13	NULL	NULL	0	NULL	torque	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intramuscular pressure was higher during isometric contraction than during eccentric and concentric activity , and the torque was in between the two latter contraction modes .
	manualset3
103495	6	401507	13	NULL	NULL	0	NULL	two 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Intramuscular pressure was higher during isometric contraction than during eccentric and concentric activity , and the torque was in between the two latter contraction modes .
	manualset3
103496	7	401507	13	NULL	NULL	0	NULL	latter contraction modes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intramuscular pressure was higher during isometric contraction than during eccentric and concentric activity , and the torque was in between the two latter contraction modes .
	manualset3
103497	1	401508	13	NULL	NULL	0	NULL	Intramuscular sincalide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Intramuscular sincalide may be useful for further studies of the value of cholecystokinin cholecystography .
	manualset3
103498	2	401508	13	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Intramuscular sincalide may be useful for further studies of the value of cholecystokinin cholecystography .
	manualset3
103499	3	401508	13	NULL	NULL	0	NULL	value 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intramuscular sincalide may be useful for further studies of the value of cholecystokinin cholecystography .
	manualset3
103500	4	401508	13	NULL	NULL	0	NULL	cholecystokinin cholecystography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Intramuscular sincalide may be useful for further studies of the value of cholecystokinin cholecystography .
	manualset3
103501	1	401509	13	NULL	NULL	0	NULL	Intranasal chlorhexidine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Intranasal chlorhexidine resulting in anaphylactic circulatory arrest .
	manualset3
103502	2	401509	13	NULL	NULL	0	NULL	anaphylactic circulatory arrest 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intranasal chlorhexidine resulting in anaphylactic circulatory arrest .
	manualset3
103503	1	401510	13	NULL	NULL	0	NULL	factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	4.1 ) and factors in subsequent delivery : birth weight ?
	manualset3
103504	2	401510	13	NULL	NULL	0	NULL	subsequent delivery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	4.1 ) and factors in subsequent delivery : birth weight ?
	manualset3
103505	3	401510	13	NULL	NULL	0	NULL	birth weight 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	4.1 ) and factors in subsequent delivery : birth weight ?
	manualset3
103506	1	401511	13	NULL	NULL	0	NULL	Intraneural ganglion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraneural ganglion of the suprascapular nerve : case report .
	manualset3
103507	2	401511	13	NULL	NULL	0	NULL	suprascapular nerve	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraneural ganglion of the suprascapular nerve : case report .
	manualset3
103508	3	401511	13	NULL	NULL	0	NULL	case report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraneural ganglion of the suprascapular nerve : case report .
	manualset3
103509	1	401512	13	NULL	NULL	0	NULL	Intraocular pressure 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraocular pressure response to medication in a clinical setting : the Marshfield Clinic Personalized Medicine Research Project .
	manualset3
103510	2	401512	13	NULL	NULL	0	NULL	 response 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraocular pressure response to medication in a clinical setting : the Marshfield Clinic Personalized Medicine Research Project .
	manualset3
103511	3	401512	13	NULL	NULL	0	NULL	medication	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraocular pressure response to medication in a clinical setting : the Marshfield Clinic Personalized Medicine Research Project .
	manualset3
103512	4	401512	13	NULL	NULL	0	NULL	clinical setting	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraocular pressure response to medication in a clinical setting : the Marshfield Clinic Personalized Medicine Research Project .
	manualset3
103513	5	401512	13	NULL	NULL	0	NULL	Marshfield Clinic Personalized Medicine Research Project	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraocular pressure response to medication in a clinical setting : the Marshfield Clinic Personalized Medicine Research Project .
	manualset3
103514	1	401513	13	NULL	NULL	0	NULL	Intraoperative complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraoperative complications include hemorrhage , microkeratome failure , flap buttonhole , dislocation , and perforation .
	manualset3
103515	2	401513	13	NULL	NULL	0	NULL	hemorrhage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraoperative complications include hemorrhage , microkeratome failure , flap buttonhole , dislocation , and perforation .
	manualset3
103516	3	401513	13	NULL	NULL	0	NULL	microkeratome failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraoperative complications include hemorrhage , microkeratome failure , flap buttonhole , dislocation , and perforation .
	manualset3
103517	4	401513	13	NULL	NULL	0	NULL	flap buttonhole	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraoperative complications include hemorrhage , microkeratome failure , flap buttonhole , dislocation , and perforation .
	manualset3
103518	5	401513	13	NULL	NULL	0	NULL	 dislocation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraoperative complications include hemorrhage , microkeratome failure , flap buttonhole , dislocation , and perforation .
	manualset3
103519	6	401513	13	NULL	NULL	0	NULL	perforation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraoperative complications include hemorrhage , microkeratome failure , flap buttonhole , dislocation , and perforation .
	manualset3
103520	1	401514	13	NULL	NULL	0	NULL	Intraoperative data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraoperative data show that 6 mm is the ideal diameter for a portacaval shunt to prompt an experimental model based on partial decompression of portal bed in animals in this size .
	manualset3
103521	2	401514	13	NULL	NULL	0	NULL	6 mm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraoperative data show that 6 mm is the ideal diameter for a portacaval shunt to prompt an experimental model based on partial decompression of portal bed in animals in this size .
	manualset3
103522	3	401514	13	NULL	NULL	0	NULL	 ideal diameter	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraoperative data show that 6 mm is the ideal diameter for a portacaval shunt to prompt an experimental model based on partial decompression of portal bed in animals in this size .
	manualset3
103523	4	401514	13	NULL	NULL	0	NULL	portacaval shunt 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraoperative data show that 6 mm is the ideal diameter for a portacaval shunt to prompt an experimental model based on partial decompression of portal bed in animals in this size .
	manualset3
103524	5	401514	13	NULL	NULL	0	NULL	experimental model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraoperative data show that 6 mm is the ideal diameter for a portacaval shunt to prompt an experimental model based on partial decompression of portal bed in animals in this size .
	manualset3
103525	6	401514	13	NULL	NULL	0	NULL	partial decompression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraoperative data show that 6 mm is the ideal diameter for a portacaval shunt to prompt an experimental model based on partial decompression of portal bed in animals in this size .
	manualset3
103526	7	401514	13	NULL	NULL	0	NULL	portal bed	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraoperative data show that 6 mm is the ideal diameter for a portacaval shunt to prompt an experimental model based on partial decompression of portal bed in animals in this size .
	manualset3
103527	8	401514	13	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraoperative data show that 6 mm is the ideal diameter for a portacaval shunt to prompt an experimental model based on partial decompression of portal bed in animals in this size .
	manualset3
103528	9	401514	13	NULL	NULL	0	NULL	size	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraoperative data show that 6 mm is the ideal diameter for a portacaval shunt to prompt an experimental model based on partial decompression of portal bed in animals in this size .
	manualset3
103529	1	401515	13	NULL	NULL	0	NULL	Intraoperative epicardial echocardiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraoperative epicardial echocardiography and color flow Doppler were performed before and after cardiopulmonary bypass in 17 consecutive patients undergoing 20 freehand allograft aortic valve replacements .
	manualset3
103530	2	401515	13	NULL	NULL	0	NULL	color flow Doppler 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraoperative epicardial echocardiography and color flow Doppler were performed before and after cardiopulmonary bypass in 17 consecutive patients undergoing 20 freehand allograft aortic valve replacements .
	manualset3
103531	3	401515	13	NULL	NULL	0	NULL	 cardiopulmonary bypass	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraoperative epicardial echocardiography and color flow Doppler were performed before and after cardiopulmonary bypass in 17 consecutive patients undergoing 20 freehand allograft aortic valve replacements .
	manualset3
103532	4	401515	13	NULL	NULL	0	NULL	 17	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraoperative epicardial echocardiography and color flow Doppler were performed before and after cardiopulmonary bypass in 17 consecutive patients undergoing 20 freehand allograft aortic valve replacements .
	manualset3
103533	5	401515	13	NULL	NULL	0	NULL	consecutive patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraoperative epicardial echocardiography and color flow Doppler were performed before and after cardiopulmonary bypass in 17 consecutive patients undergoing 20 freehand allograft aortic valve replacements .
	manualset3
103534	6	401515	13	NULL	NULL	0	NULL	20 freehand allograft aortic valve replacements 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraoperative epicardial echocardiography and color flow Doppler were performed before and after cardiopulmonary bypass in 17 consecutive patients undergoing 20 freehand allograft aortic valve replacements .
	manualset3
103535	1	401516	13	NULL	NULL	0	NULL	Intraoperative inspection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraoperative inspection of the collecting system is the most accurate method to fully define an extent of injury .
	manualset3
103536	2	401516	13	NULL	NULL	0	NULL	collecting system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraoperative inspection of the collecting system is the most accurate method to fully define an extent of injury .
	manualset3
103537	3	401516	13	NULL	NULL	0	NULL	accurate method	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraoperative inspection of the collecting system is the most accurate method to fully define an extent of injury .
	manualset3
103538	4	401516	13	NULL	NULL	0	NULL	extent of injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraoperative inspection of the collecting system is the most accurate method to fully define an extent of injury .
	manualset3
103539	1	401517	13	NULL	NULL	0	NULL	Intraoperative mild hypothermia therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraoperative mild hypothermia therapy in patients scheduled for neurosurgical procedures .
	manualset3
103540	2	401517	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraoperative mild hypothermia therapy in patients scheduled for neurosurgical procedures .
	manualset3
103541	3	401517	13	NULL	NULL	0	NULL	neurosurgical procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraoperative mild hypothermia therapy in patients scheduled for neurosurgical procedures .
	manualset3
103542	1	401518	13	NULL	NULL	0	NULL	Intraperitoneal implantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraperitoneal implantation into streptozocin ( STZ ) - induced diabetic mice was performed to investigate in vivo function of the encapsulated cells .
	manualset3
103543	2	401518	13	NULL	NULL	0	NULL	streptozocin ( STZ ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraperitoneal implantation into streptozocin ( STZ ) - induced diabetic mice was performed to investigate in vivo function of the encapsulated cells .
	manualset3
103544	3	401518	13	NULL	NULL	0	NULL	 diabetic mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraperitoneal implantation into streptozocin ( STZ ) - induced diabetic mice was performed to investigate in vivo function of the encapsulated cells .
	manualset3
103545	4	401518	13	NULL	NULL	0	NULL	in vivo function 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraperitoneal implantation into streptozocin ( STZ ) - induced diabetic mice was performed to investigate in vivo function of the encapsulated cells .
	manualset3
103546	5	401518	13	NULL	NULL	0	NULL	 encapsulated cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Intraperitoneal implantation into streptozocin ( STZ ) - induced diabetic mice was performed to investigate in vivo function of the encapsulated cells .
	manualset3
103547	1	401519	13	NULL	NULL	0	NULL	Intrathecal coadministration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intrathecal coadministration of serotonin and morphine differentially modulates the tail-flick reflex of intact and spinal rats .
	manualset3
103548	2	401519	13	NULL	NULL	0	NULL	serotonin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Intrathecal coadministration of serotonin and morphine differentially modulates the tail-flick reflex of intact and spinal rats .
	manualset3
103549	3	401519	13	NULL	NULL	0	NULL	morphine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Intrathecal coadministration of serotonin and morphine differentially modulates the tail-flick reflex of intact and spinal rats .
	manualset3
103550	4	401519	13	NULL	NULL	0	NULL	 tail-flick reflex	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intrathecal coadministration of serotonin and morphine differentially modulates the tail-flick reflex of intact and spinal rats .
	manualset3
103551	5	401519	13	NULL	NULL	0	NULL	spinal rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Intrathecal coadministration of serotonin and morphine differentially modulates the tail-flick reflex of intact and spinal rats .
	manualset3
103552	6	401519	13	NULL	NULL	0	NULL	intact rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Intrathecal coadministration of serotonin and morphine differentially modulates the tail-flick reflex of intact and spinal rats .
	manualset3
103553	1	401520	13	NULL	NULL	0	NULL	4 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	4 % ) of the lignin side chain was found to be acetylated at the gamma-carbon , predominantly over syringyl units .
	manualset3
103554	2	401520	13	NULL	NULL	0	NULL	lignin side chain	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	4 % ) of the lignin side chain was found to be acetylated at the gamma-carbon , predominantly over syringyl units .
	manualset3
103555	3	401520	13	NULL	NULL	0	NULL	gamma-carbon	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	4 % ) of the lignin side chain was found to be acetylated at the gamma-carbon , predominantly over syringyl units .
	manualset3
103556	4	401520	13	NULL	NULL	0	NULL	syringyl units	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	4 % ) of the lignin side chain was found to be acetylated at the gamma-carbon , predominantly over syringyl units .
	manualset3
103637	1	401521	13	NULL	NULL	0	NULL	Intratumor host cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Intratumor host cells of methylcholanthrene-induced fibrosarcoma ( s ) were shown to enhance the in vivo outgrowth of syngeneic homologous tumors ( MC1A , Mc2A , Mc2B ) but not two heterologous T-lymphomas ( EL4 and TLX9 ) in the Winn adoptive transfer assay .
	manualset3
103638	2	401521	13	NULL	NULL	0	NULL	methylcholanthrene-induced fibrosarcoma ( s ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intratumor host cells of methylcholanthrene-induced fibrosarcoma ( s ) were shown to enhance the in vivo outgrowth of syngeneic homologous tumors ( MC1A , Mc2A , Mc2B ) but not two heterologous T-lymphomas ( EL4 and TLX9 ) in the Winn adoptive transfer assay .
	manualset3
103639	3	401521	13	NULL	NULL	0	NULL	in vivo outgrowth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intratumor host cells of methylcholanthrene-induced fibrosarcoma ( s ) were shown to enhance the in vivo outgrowth of syngeneic homologous tumors ( MC1A , Mc2A , Mc2B ) but not two heterologous T-lymphomas ( EL4 and TLX9 ) in the Winn adoptive transfer assay .
	manualset3
103640	4	401521	13	NULL	NULL	0	NULL	 syngeneic homologous tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intratumor host cells of methylcholanthrene-induced fibrosarcoma ( s ) were shown to enhance the in vivo outgrowth of syngeneic homologous tumors ( MC1A , Mc2A , Mc2B ) but not two heterologous T-lymphomas ( EL4 and TLX9 ) in the Winn adoptive transfer assay .
	manualset3
103641	5	401521	13	NULL	NULL	0	NULL	MC1A	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intratumor host cells of methylcholanthrene-induced fibrosarcoma ( s ) were shown to enhance the in vivo outgrowth of syngeneic homologous tumors ( MC1A , Mc2A , Mc2B ) but not two heterologous T-lymphomas ( EL4 and TLX9 ) in the Winn adoptive transfer assay .
	manualset3
103642	6	401521	13	NULL	NULL	0	NULL	Mc2A	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intratumor host cells of methylcholanthrene-induced fibrosarcoma ( s ) were shown to enhance the in vivo outgrowth of syngeneic homologous tumors ( MC1A , Mc2A , Mc2B ) but not two heterologous T-lymphomas ( EL4 and TLX9 ) in the Winn adoptive transfer assay .
	manualset3
103643	7	401521	13	NULL	NULL	0	NULL	Mc2B 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intratumor host cells of methylcholanthrene-induced fibrosarcoma ( s ) were shown to enhance the in vivo outgrowth of syngeneic homologous tumors ( MC1A , Mc2A , Mc2B ) but not two heterologous T-lymphomas ( EL4 and TLX9 ) in the Winn adoptive transfer assay .
	manualset3
103644	8	401521	13	NULL	NULL	0	NULL	two heterologous T-lymphomas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intratumor host cells of methylcholanthrene-induced fibrosarcoma ( s ) were shown to enhance the in vivo outgrowth of syngeneic homologous tumors ( MC1A , Mc2A , Mc2B ) but not two heterologous T-lymphomas ( EL4 and TLX9 ) in the Winn adoptive transfer assay .
	manualset3
103645	9	401521	13	NULL	NULL	0	NULL	 EL4	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intratumor host cells of methylcholanthrene-induced fibrosarcoma ( s ) were shown to enhance the in vivo outgrowth of syngeneic homologous tumors ( MC1A , Mc2A , Mc2B ) but not two heterologous T-lymphomas ( EL4 and TLX9 ) in the Winn adoptive transfer assay .
	manualset3
103646	10	401521	13	NULL	NULL	0	NULL	TLX9	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intratumor host cells of methylcholanthrene-induced fibrosarcoma ( s ) were shown to enhance the in vivo outgrowth of syngeneic homologous tumors ( MC1A , Mc2A , Mc2B ) but not two heterologous T-lymphomas ( EL4 and TLX9 ) in the Winn adoptive transfer assay .
	manualset3
103647	11	401521	13	NULL	NULL	0	NULL	Winn adoptive transfer assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Intratumor host cells of methylcholanthrene-induced fibrosarcoma ( s ) were shown to enhance the in vivo outgrowth of syngeneic homologous tumors ( MC1A , Mc2A , Mc2B ) but not two heterologous T-lymphomas ( EL4 and TLX9 ) in the Winn adoptive transfer assay .
	manualset3
103648	1	401522	13	NULL	NULL	0	NULL	Intratumoral delivery 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Intratumoral delivery is more suitable for non-targeted modified PEI/siRNA complexes to inhibit the tumor growth in vivo .
	manualset3
103649	2	401522	13	NULL	NULL	0	NULL	PEI/siRNA complexes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Intratumoral delivery is more suitable for non-targeted modified PEI/siRNA complexes to inhibit the tumor growth in vivo .
	manualset3
103650	3	401522	13	NULL	NULL	0	NULL	 tumor growth 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intratumoral delivery is more suitable for non-targeted modified PEI/siRNA complexes to inhibit the tumor growth in vivo .
	manualset3
103651	1	401523	13	NULL	NULL	0	NULL	Intratumoral oestrone sulphatase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intratumoral oestrone sulphatase activity as a prognostic marker in human breast carcinoma .
	manualset3
103652	2	401523	13	NULL	NULL	0	NULL	prognostic marker 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intratumoral oestrone sulphatase activity as a prognostic marker in human breast carcinoma .
	manualset3
103653	3	401523	13	NULL	NULL	0	NULL	 human breast carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Intratumoral oestrone sulphatase activity as a prognostic marker in human breast carcinoma .
	manualset3
103654	1	401524	13	NULL	NULL	0	NULL	Intratympanic treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intratympanic treatment of intractable unilateral meniere disease : gentamicin or dexamethasone ?
	manualset3
103655	2	401524	13	NULL	NULL	0	NULL	meniere disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Intratympanic treatment of intractable unilateral meniere disease : gentamicin or dexamethasone ?
	manualset3
103656	3	401524	13	NULL	NULL	0	NULL	gentamicin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Intratympanic treatment of intractable unilateral meniere disease : gentamicin or dexamethasone ?
	manualset3
103657	4	401524	13	NULL	NULL	0	NULL	dexamethasone 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Intratympanic treatment of intractable unilateral meniere disease : gentamicin or dexamethasone ?
	manualset3
103658	1	401525	13	NULL	NULL	0	NULL	Intrauterine growth retardation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intrauterine growth retardation associated with hypoxia due to bronchiectasis .
	manualset3
103659	2	401525	13	NULL	NULL	0	NULL	hypoxia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intrauterine growth retardation associated with hypoxia due to bronchiectasis .
	manualset3
103660	3	401525	13	NULL	NULL	0	NULL	bronchiectasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intrauterine growth retardation associated with hypoxia due to bronchiectasis .
	manualset3
103661	1	401526	13	NULL	NULL	0	NULL	Intravascular blood coagulation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravascular blood coagulation has been shown to play the leading role in the development of hemostatic disorders with reference to 34 patients with chronic renal failure .
	manualset3
103662	2	401526	13	NULL	NULL	0	NULL	 role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravascular blood coagulation has been shown to play the leading role in the development of hemostatic disorders with reference to 34 patients with chronic renal failure .
	manualset3
103663	3	401526	13	NULL	NULL	0	NULL	development of hemostatic disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravascular blood coagulation has been shown to play the leading role in the development of hemostatic disorders with reference to 34 patients with chronic renal failure .
	manualset3
103664	4	401526	13	NULL	NULL	0	NULL	reference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravascular blood coagulation has been shown to play the leading role in the development of hemostatic disorders with reference to 34 patients with chronic renal failure .
	manualset3
103665	5	401526	13	NULL	NULL	0	NULL	34 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravascular blood coagulation has been shown to play the leading role in the development of hemostatic disorders with reference to 34 patients with chronic renal failure .
	manualset3
103666	6	401526	13	NULL	NULL	0	NULL	chronic renal failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravascular blood coagulation has been shown to play the leading role in the development of hemostatic disorders with reference to 34 patients with chronic renal failure .
	manualset3
103667	1	401527	13	NULL	NULL	0	NULL	Intravascular fetal transfusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravascular fetal transfusion can be complicated by difficulty in maintaining vascular access because of fetal movements .
	manualset3
103668	2	401527	13	NULL	NULL	0	NULL	difficulty	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravascular fetal transfusion can be complicated by difficulty in maintaining vascular access because of fetal movements .
	manualset3
103669	3	401527	13	NULL	NULL	0	NULL	vascular access	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravascular fetal transfusion can be complicated by difficulty in maintaining vascular access because of fetal movements .
	manualset3
103670	4	401527	13	NULL	NULL	0	NULL	fetal movements	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravascular fetal transfusion can be complicated by difficulty in maintaining vascular access because of fetal movements .
	manualset3
103671	1	401528	13	NULL	NULL	0	NULL	Intravenous bolus injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous bolus injection of increasing doses of MIBG up to 400 nmol resulted in a significant ( F ratio = 7.778 , P less than 0.0001 ) dose dependent decrease of MIBG extraction in both awake and anaesthetised sheep , without significant differences of extraction values between the two groups .
	manualset3
103672	2	401528	13	NULL	NULL	NULL	NULL	doses of MIBG	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Intravenous bolus injection of increasing doses of MIBG up to 400 nmol resulted in a significant ( F ratio = 7.778 , P less than 0.0001 ) dose dependent decrease of MIBG extraction in both awake and anaesthetised sheep , without significant differences of extraction values between the two groups .
	manualset3
103673	3	401528	13	NULL	NULL	0	NULL	 400 nmol 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous bolus injection of increasing doses of MIBG up to 400 nmol resulted in a significant ( F ratio = 7.778 , P less than 0.0001 ) dose dependent decrease of MIBG extraction in both awake and anaesthetised sheep , without significant differences of extraction values between the two groups .
	manualset3
103674	4	401528	13	NULL	NULL	0	NULL	F ratio = 7.778 , P less than 0.0001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous bolus injection of increasing doses of MIBG up to 400 nmol resulted in a significant ( F ratio = 7.778 , P less than 0.0001 ) dose dependent decrease of MIBG extraction in both awake and anaesthetised sheep , without significant differences of extraction values between the two groups .
	manualset3
103675	5	401528	13	NULL	NULL	0	NULL	 dose	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous bolus injection of increasing doses of MIBG up to 400 nmol resulted in a significant ( F ratio = 7.778 , P less than 0.0001 ) dose dependent decrease of MIBG extraction in both awake and anaesthetised sheep , without significant differences of extraction values between the two groups .
	manualset3
103676	6	401528	13	NULL	NULL	0	NULL	decrease of MIBG extraction 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous bolus injection of increasing doses of MIBG up to 400 nmol resulted in a significant ( F ratio = 7.778 , P less than 0.0001 ) dose dependent decrease of MIBG extraction in both awake and anaesthetised sheep , without significant differences of extraction values between the two groups .
	manualset3
103677	7	401528	13	NULL	NULL	0	NULL	awake sheep	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous bolus injection of increasing doses of MIBG up to 400 nmol resulted in a significant ( F ratio = 7.778 , P less than 0.0001 ) dose dependent decrease of MIBG extraction in both awake and anaesthetised sheep , without significant differences of extraction values between the two groups .
	manualset3
103678	8	401528	13	NULL	NULL	0	NULL	anaesthetised sheep	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous bolus injection of increasing doses of MIBG up to 400 nmol resulted in a significant ( F ratio = 7.778 , P less than 0.0001 ) dose dependent decrease of MIBG extraction in both awake and anaesthetised sheep , without significant differences of extraction values between the two groups .
	manualset3
103679	9	401528	13	NULL	NULL	0	NULL	differences of extraction values 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous bolus injection of increasing doses of MIBG up to 400 nmol resulted in a significant ( F ratio = 7.778 , P less than 0.0001 ) dose dependent decrease of MIBG extraction in both awake and anaesthetised sheep , without significant differences of extraction values between the two groups .
	manualset3
103680	10	401528	13	NULL	NULL	0	NULL	 two groups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous bolus injection of increasing doses of MIBG up to 400 nmol resulted in a significant ( F ratio = 7.778 , P less than 0.0001 ) dose dependent decrease of MIBG extraction in both awake and anaesthetised sheep , without significant differences of extraction values between the two groups .
	manualset3
103681	1	401529	13	NULL	NULL	0	NULL	admission Barthel index score 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	4 ) The higher the admission Barthel index score , the shorter the period of stay ( p less than 0.01 ) .
	manualset3
103682	2	401529	13	NULL	NULL	0	NULL	period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	4 ) The higher the admission Barthel index score , the shorter the period of stay ( p less than 0.01 ) .
	manualset3
103683	3	401529	13	NULL	NULL	0	NULL	stay	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	4 ) The higher the admission Barthel index score , the shorter the period of stay ( p less than 0.01 ) .
	manualset3
103684	4	401529	13	NULL	NULL	0	NULL	p less than 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	4 ) The higher the admission Barthel index score , the shorter the period of stay ( p less than 0.01 ) .
	manualset3
103685	1	401530	13	NULL	NULL	0	NULL	Intravenous infusion 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous infusion of ANP ( 1 or 5 micrograms/h ) or of isotonic saline ( 2 or 4 ml/h ) did not alter urinary kallikrein output .
	manualset3
103686	2	401530	13	NULL	NULL	0	NULL	ANP	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous infusion of ANP ( 1 or 5 micrograms/h ) or of isotonic saline ( 2 or 4 ml/h ) did not alter urinary kallikrein output .
	manualset3
103687	3	401530	13	NULL	NULL	0	NULL	1 or 5 micrograms/h 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous infusion of ANP ( 1 or 5 micrograms/h ) or of isotonic saline ( 2 or 4 ml/h ) did not alter urinary kallikrein output .
	manualset3
103688	4	401530	13	NULL	NULL	0	NULL	isotonic saline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous infusion of ANP ( 1 or 5 micrograms/h ) or of isotonic saline ( 2 or 4 ml/h ) did not alter urinary kallikrein output .
	manualset3
103689	5	401530	13	NULL	NULL	0	NULL	 2 or 4 ml/h	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous infusion of ANP ( 1 or 5 micrograms/h ) or of isotonic saline ( 2 or 4 ml/h ) did not alter urinary kallikrein output .
	manualset3
103690	6	401530	13	NULL	NULL	0	NULL	urinary kallikrein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous infusion of ANP ( 1 or 5 micrograms/h ) or of isotonic saline ( 2 or 4 ml/h ) did not alter urinary kallikrein output .
	manualset3
103691	7	401530	13	NULL	NULL	0	NULL	output	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous infusion of ANP ( 1 or 5 micrograms/h ) or of isotonic saline ( 2 or 4 ml/h ) did not alter urinary kallikrein output .
	manualset3
103692	1	401531	13	NULL	NULL	0	NULL	Intravenous injection 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous injection of prazosin ( alpha 1-antagonist , 150 micrograms/kg , n = 7 ) and of yohimbine ( alpha 2-antagonist , 30 micrograms/kg , n = 7 ) decreased MCP significantly from 9.9 + / - 0.4 to 8.2 + / - 0.5 mmHg ( -17.2 % , p less than 0.01 ) , and from 9.8 + / - 0.2 to 7.6 + / - 0.3 mmHg ( -22.4 % , p less than 0.01 ) , respectively .
	manualset3
103693	2	401531	13	NULL	NULL	0	NULL	prazosin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous injection of prazosin ( alpha 1-antagonist , 150 micrograms/kg , n = 7 ) and of yohimbine ( alpha 2-antagonist , 30 micrograms/kg , n = 7 ) decreased MCP significantly from 9.9 + / - 0.4 to 8.2 + / - 0.5 mmHg ( -17.2 % , p less than 0.01 ) , and from 9.8 + / - 0.2 to 7.6 + / - 0.3 mmHg ( -22.4 % , p less than 0.01 ) , respectively .
	manualset3
103694	3	401531	13	NULL	NULL	0	NULL	alpha 1-antagonist 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous injection of prazosin ( alpha 1-antagonist , 150 micrograms/kg , n = 7 ) and of yohimbine ( alpha 2-antagonist , 30 micrograms/kg , n = 7 ) decreased MCP significantly from 9.9 + / - 0.4 to 8.2 + / - 0.5 mmHg ( -17.2 % , p less than 0.01 ) , and from 9.8 + / - 0.2 to 7.6 + / - 0.3 mmHg ( -22.4 % , p less than 0.01 ) , respectively .
	manualset3
103695	4	401531	13	NULL	NULL	0	NULL	 150 micrograms/kg , n = 7	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous injection of prazosin ( alpha 1-antagonist , 150 micrograms/kg , n = 7 ) and of yohimbine ( alpha 2-antagonist , 30 micrograms/kg , n = 7 ) decreased MCP significantly from 9.9 + / - 0.4 to 8.2 + / - 0.5 mmHg ( -17.2 % , p less than 0.01 ) , and from 9.8 + / - 0.2 to 7.6 + / - 0.3 mmHg ( -22.4 % , p less than 0.01 ) , respectively .
	manualset3
103696	5	401531	13	NULL	NULL	0	NULL	yohimbine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous injection of prazosin ( alpha 1-antagonist , 150 micrograms/kg , n = 7 ) and of yohimbine ( alpha 2-antagonist , 30 micrograms/kg , n = 7 ) decreased MCP significantly from 9.9 + / - 0.4 to 8.2 + / - 0.5 mmHg ( -17.2 % , p less than 0.01 ) , and from 9.8 + / - 0.2 to 7.6 + / - 0.3 mmHg ( -22.4 % , p less than 0.01 ) , respectively .
	manualset3
103697	6	401531	13	NULL	NULL	0	NULL	 alpha 2-antagonist	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous injection of prazosin ( alpha 1-antagonist , 150 micrograms/kg , n = 7 ) and of yohimbine ( alpha 2-antagonist , 30 micrograms/kg , n = 7 ) decreased MCP significantly from 9.9 + / - 0.4 to 8.2 + / - 0.5 mmHg ( -17.2 % , p less than 0.01 ) , and from 9.8 + / - 0.2 to 7.6 + / - 0.3 mmHg ( -22.4 % , p less than 0.01 ) , respectively .
	manualset3
103698	7	401531	13	NULL	NULL	0	NULL	30 micrograms/kg , n = 7 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous injection of prazosin ( alpha 1-antagonist , 150 micrograms/kg , n = 7 ) and of yohimbine ( alpha 2-antagonist , 30 micrograms/kg , n = 7 ) decreased MCP significantly from 9.9 + / - 0.4 to 8.2 + / - 0.5 mmHg ( -17.2 % , p less than 0.01 ) , and from 9.8 + / - 0.2 to 7.6 + / - 0.3 mmHg ( -22.4 % , p less than 0.01 ) , respectively .
	manualset3
103699	8	401531	13	NULL	NULL	0	NULL	MCP	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous injection of prazosin ( alpha 1-antagonist , 150 micrograms/kg , n = 7 ) and of yohimbine ( alpha 2-antagonist , 30 micrograms/kg , n = 7 ) decreased MCP significantly from 9.9 + / - 0.4 to 8.2 + / - 0.5 mmHg ( -17.2 % , p less than 0.01 ) , and from 9.8 + / - 0.2 to 7.6 + / - 0.3 mmHg ( -22.4 % , p less than 0.01 ) , respectively .
	manualset3
103700	9	401531	13	NULL	NULL	0	NULL	9.9 + / - 0.4 to 8.2 + / - 0.5 mmHg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous injection of prazosin ( alpha 1-antagonist , 150 micrograms/kg , n = 7 ) and of yohimbine ( alpha 2-antagonist , 30 micrograms/kg , n = 7 ) decreased MCP significantly from 9.9 + / - 0.4 to 8.2 + / - 0.5 mmHg ( -17.2 % , p less than 0.01 ) , and from 9.8 + / - 0.2 to 7.6 + / - 0.3 mmHg ( -22.4 % , p less than 0.01 ) , respectively .
	manualset3
103701	10	401531	13	NULL	NULL	0	NULL	-17.2 % , p less than 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous injection of prazosin ( alpha 1-antagonist , 150 micrograms/kg , n = 7 ) and of yohimbine ( alpha 2-antagonist , 30 micrograms/kg , n = 7 ) decreased MCP significantly from 9.9 + / - 0.4 to 8.2 + / - 0.5 mmHg ( -17.2 % , p less than 0.01 ) , and from 9.8 + / - 0.2 to 7.6 + / - 0.3 mmHg ( -22.4 % , p less than 0.01 ) , respectively .
	manualset3
103702	11	401531	13	NULL	NULL	0	NULL	9.8 + / - 0.2 to 7.6 + / - 0.3 mmHg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous injection of prazosin ( alpha 1-antagonist , 150 micrograms/kg , n = 7 ) and of yohimbine ( alpha 2-antagonist , 30 micrograms/kg , n = 7 ) decreased MCP significantly from 9.9 + / - 0.4 to 8.2 + / - 0.5 mmHg ( -17.2 % , p less than 0.01 ) , and from 9.8 + / - 0.2 to 7.6 + / - 0.3 mmHg ( -22.4 % , p less than 0.01 ) , respectively .
	manualset3
103703	12	401531	13	NULL	NULL	0	NULL	 -22.4 % , p less than 0.01 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous injection of prazosin ( alpha 1-antagonist , 150 micrograms/kg , n = 7 ) and of yohimbine ( alpha 2-antagonist , 30 micrograms/kg , n = 7 ) decreased MCP significantly from 9.9 + / - 0.4 to 8.2 + / - 0.5 mmHg ( -17.2 % , p less than 0.01 ) , and from 9.8 + / - 0.2 to 7.6 + / - 0.3 mmHg ( -22.4 % , p less than 0.01 ) , respectively .
	manualset3
104038	1	401532	13	NULL	NULL	0	NULL	Intravenous injections 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous injections of betamethasone ( 0.8 microgram/g body wt . )
	manualset3
104039	2	401532	13	NULL	NULL	0	NULL	betamethasone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous injections of betamethasone ( 0.8 microgram/g body wt . )
	manualset3
104040	3	401532	13	NULL	NULL	0	NULL	0.8 microgram/g body wt 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous injections of betamethasone ( 0.8 microgram/g body wt . )
	manualset3
104041	1	401533	13	NULL	NULL	0	NULL	Intravenous ranitidine	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous ranitidine reduces the risk of acid aspiration of gastric contents at emergency cesarean section .
	manualset3
104042	2	401533	13	NULL	NULL	0	NULL	 risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous ranitidine reduces the risk of acid aspiration of gastric contents at emergency cesarean section .
	manualset3
104043	3	401533	13	NULL	NULL	0	NULL	acid aspiration of gastric contents 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous ranitidine reduces the risk of acid aspiration of gastric contents at emergency cesarean section .
	manualset3
104044	4	401533	13	NULL	NULL	0	NULL	emergency cesarean section	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous ranitidine reduces the risk of acid aspiration of gastric contents at emergency cesarean section .
	manualset3
104045	1	401534	13	NULL	NULL	NULL	NULL	methyl-14C ) choline chloride	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Intravenously administered ( methyl-14C ) choline chloride is maximally incorporated into alveolar surface surfactant 8 h after injection , and more than 97 % of this radiolabel is present in the phosphatidylcholine fraction of the surfactant and , of this , 75 % is associated with the dipalmitoyl phosphatidylcholine species .
	manualset3
104046	2	401534	13	NULL	NULL	NULL	NULL	alveolar surface surfactant 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Intravenously administered ( methyl-14C ) choline chloride is maximally incorporated into alveolar surface surfactant 8 h after injection , and more than 97 % of this radiolabel is present in the phosphatidylcholine fraction of the surfactant and , of this , 75 % is associated with the dipalmitoyl phosphatidylcholine species .
	manualset3
104047	3	401534	13	NULL	NULL	0	NULL	8 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenously administered ( methyl-14C ) choline chloride is maximally incorporated into alveolar surface surfactant 8 h after injection , and more than 97 % of this radiolabel is present in the phosphatidylcholine fraction of the surfactant and , of this , 75 % is associated with the dipalmitoyl phosphatidylcholine species .
	manualset3
104048	4	401534	13	NULL	NULL	0	NULL	 injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenously administered ( methyl-14C ) choline chloride is maximally incorporated into alveolar surface surfactant 8 h after injection , and more than 97 % of this radiolabel is present in the phosphatidylcholine fraction of the surfactant and , of this , 75 % is associated with the dipalmitoyl phosphatidylcholine species .
	manualset3
104049	5	401534	13	NULL	NULL	0	NULL	97 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenously administered ( methyl-14C ) choline chloride is maximally incorporated into alveolar surface surfactant 8 h after injection , and more than 97 % of this radiolabel is present in the phosphatidylcholine fraction of the surfactant and , of this , 75 % is associated with the dipalmitoyl phosphatidylcholine species .
	manualset3
104050	6	401534	13	NULL	NULL	0	NULL	radiolabel 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenously administered ( methyl-14C ) choline chloride is maximally incorporated into alveolar surface surfactant 8 h after injection , and more than 97 % of this radiolabel is present in the phosphatidylcholine fraction of the surfactant and , of this , 75 % is associated with the dipalmitoyl phosphatidylcholine species .
	manualset3
104051	7	401534	13	NULL	NULL	0	NULL	phosphatidylcholine fraction	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenously administered ( methyl-14C ) choline chloride is maximally incorporated into alveolar surface surfactant 8 h after injection , and more than 97 % of this radiolabel is present in the phosphatidylcholine fraction of the surfactant and , of this , 75 % is associated with the dipalmitoyl phosphatidylcholine species .
	manualset3
104052	8	401534	13	NULL	NULL	0	NULL	surfactant	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenously administered ( methyl-14C ) choline chloride is maximally incorporated into alveolar surface surfactant 8 h after injection , and more than 97 % of this radiolabel is present in the phosphatidylcholine fraction of the surfactant and , of this , 75 % is associated with the dipalmitoyl phosphatidylcholine species .
	manualset3
104053	9	401534	13	NULL	NULL	0	NULL	75 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenously administered ( methyl-14C ) choline chloride is maximally incorporated into alveolar surface surfactant 8 h after injection , and more than 97 % of this radiolabel is present in the phosphatidylcholine fraction of the surfactant and , of this , 75 % is associated with the dipalmitoyl phosphatidylcholine species .
	manualset3
104054	10	401534	13	NULL	NULL	0	NULL	 dipalmitoyl phosphatidylcholine species 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenously administered ( methyl-14C ) choline chloride is maximally incorporated into alveolar surface surfactant 8 h after injection , and more than 97 % of this radiolabel is present in the phosphatidylcholine fraction of the surfactant and , of this , 75 % is associated with the dipalmitoyl phosphatidylcholine species .
	manualset3
104055	1	401535	13	NULL	NULL	0	NULL	3-O - methylfructose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenously infused 3-O - methylfructose produces marked 3-O - methylfructosemia without concomitant hyperglycemia ; in such animals the intestinal transport of both fructose and 3-O - methylfructose increased .
	manualset3
104057	2	401535	13	NULL	NULL	0	NULL	3-O - methylfructosemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenously infused 3-O - methylfructose produces marked 3-O - methylfructosemia without concomitant hyperglycemia ; in such animals the intestinal transport of both fructose and 3-O - methylfructose increased .
	manualset3
104058	3	401535	13	NULL	NULL	0	NULL	concomitant hyperglycemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenously infused 3-O - methylfructose produces marked 3-O - methylfructosemia without concomitant hyperglycemia ; in such animals the intestinal transport of both fructose and 3-O - methylfructose increased .
	manualset3
104060	4	401535	13	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenously infused 3-O - methylfructose produces marked 3-O - methylfructosemia without concomitant hyperglycemia ; in such animals the intestinal transport of both fructose and 3-O - methylfructose increased .
	manualset3
104061	5	401535	13	NULL	NULL	0	NULL	intestinal transport	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenously infused 3-O - methylfructose produces marked 3-O - methylfructosemia without concomitant hyperglycemia ; in such animals the intestinal transport of both fructose and 3-O - methylfructose increased .
	manualset3
104062	6	401535	13	NULL	NULL	0	NULL	fructose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenously infused 3-O - methylfructose produces marked 3-O - methylfructosemia without concomitant hyperglycemia ; in such animals the intestinal transport of both fructose and 3-O - methylfructose increased .
	manualset3
104064	7	401535	13	NULL	NULL	0	NULL	3-O - methylfructose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenously infused 3-O - methylfructose produces marked 3-O - methylfructosemia without concomitant hyperglycemia ; in such animals the intestinal transport of both fructose and 3-O - methylfructose increased .
	manualset3
104071	1	401536	13	NULL	NULL	0	NULL	( 1 , 2-3H ) deoxycorticosterone ( DOC )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenously injected ( 1 , 2-3H ) deoxycorticosterone ( DOC ) readily enters all parts of the central nervous system .
	manualset3
104072	2	401536	13	NULL	NULL	0	NULL	all parts of the central nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenously injected ( 1 , 2-3H ) deoxycorticosterone ( DOC ) readily enters all parts of the central nervous system .
	manualset3
104076	1	401537	13	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Intrigued by this hypothesis , we constructed a model for the Neurospora circadian clock , which includes expression of the frq and the wc-1 genes and their possible interactions .
	manualset3
104078	2	401537	13	NULL	NULL	0	NULL	 model for the Neurospora circadian clock	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Intrigued by this hypothesis , we constructed a model for the Neurospora circadian clock , which includes expression of the frq and the wc-1 genes and their possible interactions .
	manualset3
104079	3	401537	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intrigued by this hypothesis , we constructed a model for the Neurospora circadian clock , which includes expression of the frq and the wc-1 genes and their possible interactions .
	manualset3
104080	4	401537	13	NULL	NULL	0	NULL	frq gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Intrigued by this hypothesis , we constructed a model for the Neurospora circadian clock , which includes expression of the frq and the wc-1 genes and their possible interactions .
	manualset3
104082	5	401537	13	NULL	NULL	0	NULL	wc-1 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Intrigued by this hypothesis , we constructed a model for the Neurospora circadian clock , which includes expression of the frq and the wc-1 genes and their possible interactions .
	manualset3
104083	6	401537	13	NULL	NULL	0	NULL	interactions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intrigued by this hypothesis , we constructed a model for the Neurospora circadian clock , which includes expression of the frq and the wc-1 genes and their possible interactions .
	manualset3
104089	1	401538	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Intriguingly , our results suggest that TF binding and HMs are redundant in strict statistical sense for predicting gene expression .
	manualset3
104090	2	401538	13	NULL	NULL	0	NULL	TF binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intriguingly , our results suggest that TF binding and HMs are redundant in strict statistical sense for predicting gene expression .
	manualset3
104094	3	401538	13	NULL	NULL	0	NULL	HMs	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intriguingly , our results suggest that TF binding and HMs are redundant in strict statistical sense for predicting gene expression .
	manualset3
104096	4	401538	13	NULL	NULL	0	NULL	statistical sense	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Intriguingly , our results suggest that TF binding and HMs are redundant in strict statistical sense for predicting gene expression .
	manualset3
104099	5	401538	13	NULL	NULL	0	NULL	gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intriguingly , our results suggest that TF binding and HMs are redundant in strict statistical sense for predicting gene expression .
	manualset3
104101	1	401539	13	NULL	NULL	0	NULL	basal diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	4 , the basal diet was supplemented as in Exp .
	manualset3
104102	2	401539	13	NULL	NULL	0	NULL	Exp 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	4 , the basal diet was supplemented as in Exp .
	manualset3
104104	1	401540	13	NULL	NULL	0	NULL	activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intriguingly , the activities of these proteins are interdependent ; MdmX stabilizes Mdm2 , enabling its activities towards p53 , but it also requires Mdm2 for its nuclear localization .
	manualset3
104105	2	401540	13	NULL	NULL	0	NULL	proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Intriguingly , the activities of these proteins are interdependent ; MdmX stabilizes Mdm2 , enabling its activities towards p53 , but it also requires Mdm2 for its nuclear localization .
	manualset3
104106	3	401540	13	NULL	NULL	0	NULL	MdmX	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Intriguingly , the activities of these proteins are interdependent ; MdmX stabilizes Mdm2 , enabling its activities towards p53 , but it also requires Mdm2 for its nuclear localization .
	manualset3
104107	4	401540	13	NULL	NULL	0	NULL	Mdm2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Intriguingly , the activities of these proteins are interdependent ; MdmX stabilizes Mdm2 , enabling its activities towards p53 , but it also requires Mdm2 for its nuclear localization .
	manualset3
104109	5	401540	13	NULL	NULL	0	NULL	activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intriguingly , the activities of these proteins are interdependent ; MdmX stabilizes Mdm2 , enabling its activities towards p53 , but it also requires Mdm2 for its nuclear localization .
	manualset3
104110	6	401540	13	NULL	NULL	0	NULL	p53 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Intriguingly , the activities of these proteins are interdependent ; MdmX stabilizes Mdm2 , enabling its activities towards p53 , but it also requires Mdm2 for its nuclear localization .
	manualset3
104112	7	401540	13	NULL	NULL	0	NULL	Mdm2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Intriguingly , the activities of these proteins are interdependent ; MdmX stabilizes Mdm2 , enabling its activities towards p53 , but it also requires Mdm2 for its nuclear localization .
	manualset3
104114	8	401540	13	NULL	NULL	0	NULL	 nuclear localization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intriguingly , the activities of these proteins are interdependent ; MdmX stabilizes Mdm2 , enabling its activities towards p53 , but it also requires Mdm2 for its nuclear localization .
	manualset3
104149	1	401541	13	NULL	NULL	0	NULL	Intrinsic function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intrinsic function of a neuronal network - a vertebrate central pattern generator .
	manualset3
104150	2	401541	13	NULL	NULL	0	NULL	neuronal network	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intrinsic function of a neuronal network - a vertebrate central pattern generator .
	manualset3
104151	3	401541	13	NULL	NULL	0	NULL	vertebrate central pattern generator	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intrinsic function of a neuronal network - a vertebrate central pattern generator .
	manualset3
104152	1	401542	13	NULL	NULL	0	NULL	human lysozyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Introducing human lysozyme into pigs ' milk has a potential to benefit the piglets by enhancing immune function and defending against pathogenic bacteria , thereby increasing the new born survival rate .
	manualset3
104153	2	401542	13	NULL	NULL	0	NULL	pigs ' milk 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Introducing human lysozyme into pigs ' milk has a potential to benefit the piglets by enhancing immune function and defending against pathogenic bacteria , thereby increasing the new born survival rate .
	manualset3
104154	3	401542	13	NULL	NULL	0	NULL	 piglets	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Introducing human lysozyme into pigs ' milk has a potential to benefit the piglets by enhancing immune function and defending against pathogenic bacteria , thereby increasing the new born survival rate .
	manualset3
104155	4	401542	13	NULL	NULL	0	NULL	immune function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Introducing human lysozyme into pigs ' milk has a potential to benefit the piglets by enhancing immune function and defending against pathogenic bacteria , thereby increasing the new born survival rate .
	manualset3
104156	5	401542	13	NULL	NULL	0	NULL	pathogenic bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Introducing human lysozyme into pigs ' milk has a potential to benefit the piglets by enhancing immune function and defending against pathogenic bacteria , thereby increasing the new born survival rate .
	manualset3
104157	6	401542	13	NULL	NULL	0	NULL	new born survival rate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Introducing human lysozyme into pigs ' milk has a potential to benefit the piglets by enhancing immune function and defending against pathogenic bacteria , thereby increasing the new born survival rate .
	manualset3
104162	1	401543	13	NULL	NULL	0	NULL	microcomputers	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Introducing microcomputers : anticipating the problems .
	manualset3
104163	2	401543	13	NULL	NULL	0	NULL	problems	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Introducing microcomputers : anticipating the problems .
	manualset3
104165	1	401544	13	NULL	NULL	0	NULL	Introduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Introduction : diet , epigenetic events and cancer prevention .
	manualset3
104167	2	401544	13	NULL	NULL	0	NULL	diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Introduction : diet , epigenetic events and cancer prevention .
	manualset3
104169	3	401544	13	NULL	NULL	0	NULL	epigenetic events	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Introduction : diet , epigenetic events and cancer prevention .
	manualset3
104170	4	401544	13	NULL	NULL	0	NULL	cancer prevention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Introduction : diet , epigenetic events and cancer prevention .
	manualset3
104184	1	401545	13	NULL	NULL	0	NULL	Introduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Introduction of methyl groups at the 3 and 5positions on the pyridyl unit diminishes the non-radiative rate constant by locking the peripheral pyridyl group orthogonally to the dipyrrinato plane .
	manualset3
104185	2	401545	13	NULL	NULL	0	NULL	methyl groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Introduction of methyl groups at the 3 and 5positions on the pyridyl unit diminishes the non-radiative rate constant by locking the peripheral pyridyl group orthogonally to the dipyrrinato plane .
	manualset3
104186	3	401545	13	NULL	NULL	0	NULL	3 position 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Introduction of methyl groups at the 3 and 5positions on the pyridyl unit diminishes the non-radiative rate constant by locking the peripheral pyridyl group orthogonally to the dipyrrinato plane .
	manualset3
104188	4	401545	13	NULL	NULL	0	NULL	5position	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Introduction of methyl groups at the 3 and 5positions on the pyridyl unit diminishes the non-radiative rate constant by locking the peripheral pyridyl group orthogonally to the dipyrrinato plane .
	manualset3
104197	5	401545	13	NULL	NULL	0	NULL	pyridyl unit	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Introduction of methyl groups at the 3 and 5positions on the pyridyl unit diminishes the non-radiative rate constant by locking the peripheral pyridyl group orthogonally to the dipyrrinato plane .
	manualset3
104199	6	401545	13	NULL	NULL	0	NULL	non-radiative rate constant	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Introduction of methyl groups at the 3 and 5positions on the pyridyl unit diminishes the non-radiative rate constant by locking the peripheral pyridyl group orthogonally to the dipyrrinato plane .
	manualset3
104201	7	401545	13	NULL	NULL	0	NULL	peripheral pyridyl group 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Introduction of methyl groups at the 3 and 5positions on the pyridyl unit diminishes the non-radiative rate constant by locking the peripheral pyridyl group orthogonally to the dipyrrinato plane .
	manualset3
104204	8	401545	13	NULL	NULL	0	NULL	dipyrrinato plane	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Introduction of methyl groups at the 3 and 5positions on the pyridyl unit diminishes the non-radiative rate constant by locking the peripheral pyridyl group orthogonally to the dipyrrinato plane .
	manualset3
104205	1	401546	13	NULL	NULL	0	NULL	Introduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Introduction of potential sex factors into Rhizobium japonicum .
	manualset3
104206	2	401546	13	NULL	NULL	0	NULL	potential sex factors	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Introduction of potential sex factors into Rhizobium japonicum .
	manualset3
104207	3	401546	13	NULL	NULL	0	NULL	 Rhizobium japonicum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Introduction of potential sex factors into Rhizobium japonicum .
	manualset3
104208	1	401547	13	NULL	NULL	0	NULL	Introduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Introduction of the intramedullary bone block has reduced the revision rate for stem loosening to less than 1 % at 14 years and completely eliminated stem fracture .
	manualset3
104209	2	401547	13	NULL	NULL	0	NULL	intramedullary bone block	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Introduction of the intramedullary bone block has reduced the revision rate for stem loosening to less than 1 % at 14 years and completely eliminated stem fracture .
	manualset3
104210	3	401547	13	NULL	NULL	0	NULL	revision rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Introduction of the intramedullary bone block has reduced the revision rate for stem loosening to less than 1 % at 14 years and completely eliminated stem fracture .
	manualset3
104211	4	401547	13	NULL	NULL	0	NULL	stem	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Introduction of the intramedullary bone block has reduced the revision rate for stem loosening to less than 1 % at 14 years and completely eliminated stem fracture .
	manualset3
104212	5	401547	13	NULL	NULL	0	NULL	less than 1 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Introduction of the intramedullary bone block has reduced the revision rate for stem loosening to less than 1 % at 14 years and completely eliminated stem fracture .
	manualset3
104213	6	401547	13	NULL	NULL	0	NULL	14 years	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Introduction of the intramedullary bone block has reduced the revision rate for stem loosening to less than 1 % at 14 years and completely eliminated stem fracture .
	manualset3
104214	7	401547	13	NULL	NULL	0	NULL	stem fracture 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Introduction of the intramedullary bone block has reduced the revision rate for stem loosening to less than 1 % at 14 years and completely eliminated stem fracture .
	manualset3
104215	1	401548	13	NULL	NULL	0	NULL	Introduction strategy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Introduction strategy of a second dose measles containing vaccine in India .
	manualset3
104216	2	401548	13	NULL	NULL	0	NULL	second dose	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Introduction strategy of a second dose measles containing vaccine in India .
	manualset3
104217	3	401548	13	NULL	NULL	0	NULL	measles	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Introduction strategy of a second dose measles containing vaccine in India .
	manualset3
104218	4	401548	13	NULL	NULL	0	NULL	vaccine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Introduction strategy of a second dose measles containing vaccine in India .
	manualset3
104219	5	401548	13	NULL	NULL	0	NULL	India	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Introduction strategy of a second dose measles containing vaccine in India .
	manualset3
104220	1	401549	13	NULL	NULL	0	NULL	Introduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	IntroductionRadioactive contamination can occur as a result of accidental or intentional release of radioactive materials ( RM ) into the environment .
	manualset3
104221	2	401549	13	NULL	NULL	0	NULL	Radioactive contamination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	IntroductionRadioactive contamination can occur as a result of accidental or intentional release of radioactive materials ( RM ) into the environment .
	manualset3
104222	3	401549	13	NULL	NULL	NULL	NULL	 result 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	IntroductionRadioactive contamination can occur as a result of accidental or intentional release of radioactive materials ( RM ) into the environment .
	manualset3
104223	4	401549	13	NULL	NULL	0	NULL	accidental release	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	IntroductionRadioactive contamination can occur as a result of accidental or intentional release of radioactive materials ( RM ) into the environment .
	manualset3
104224	5	401549	13	NULL	NULL	0	NULL	 intentional release	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	IntroductionRadioactive contamination can occur as a result of accidental or intentional release of radioactive materials ( RM ) into the environment .
	manualset3
104225	6	401549	13	NULL	NULL	0	NULL	radioactive materials ( RM )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	IntroductionRadioactive contamination can occur as a result of accidental or intentional release of radioactive materials ( RM ) into the environment .
	manualset3
104226	7	401549	13	NULL	NULL	0	NULL	environment 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	IntroductionRadioactive contamination can occur as a result of accidental or intentional release of radioactive materials ( RM ) into the environment .
	manualset3
104227	1	401550	13	NULL	NULL	0	NULL	basement membrane matrix 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Invading basement membrane matrix is sufficient for MDA-MB-231 breast cancer cells to develop a stable in vivo metastatic phenotype .
	manualset3
104228	2	401550	13	NULL	NULL	0	NULL	 MDA-MB-231 breast cancer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Invading basement membrane matrix is sufficient for MDA-MB-231 breast cancer cells to develop a stable in vivo metastatic phenotype .
	manualset3
104229	3	401550	13	NULL	NULL	0	NULL	stable	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Invading basement membrane matrix is sufficient for MDA-MB-231 breast cancer cells to develop a stable in vivo metastatic phenotype .
	manualset3
104230	4	401550	13	NULL	NULL	NULL	NULL	in vivo metastatic phenotype 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Invading basement membrane matrix is sufficient for MDA-MB-231 breast cancer cells to develop a stable in vivo metastatic phenotype .
	manualset3
104231	1	401551	13	NULL	NULL	0	NULL	Invasion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Invasion of an untwisted dsDNA by a nucleoprotein filament leads to an exchanged duplex that remains topologically linked to the exchanged single strand , suggesting multiple initiations of strand exchange on the same molecule .
	manualset3
104232	2	401551	13	NULL	NULL	0	NULL	dsDNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Invasion of an untwisted dsDNA by a nucleoprotein filament leads to an exchanged duplex that remains topologically linked to the exchanged single strand , suggesting multiple initiations of strand exchange on the same molecule .
	manualset3
104233	3	401551	13	NULL	NULL	0	NULL	nucleoprotein filament 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Invasion of an untwisted dsDNA by a nucleoprotein filament leads to an exchanged duplex that remains topologically linked to the exchanged single strand , suggesting multiple initiations of strand exchange on the same molecule .
	manualset3
104234	4	401551	13	NULL	NULL	0	NULL	 single strand	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Invasion of an untwisted dsDNA by a nucleoprotein filament leads to an exchanged duplex that remains topologically linked to the exchanged single strand , suggesting multiple initiations of strand exchange on the same molecule .
	manualset3
104235	4	401551	13	NULL	NULL	NULL	NULL	multiple initiations	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Invasion of an untwisted dsDNA by a nucleoprotein filament leads to an exchanged duplex that remains topologically linked to the exchanged single strand , suggesting multiple initiations of strand exchange on the same molecule .
	manualset3
104236	5	401551	13	NULL	NULL	0	NULL	strand exchange	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Invasion of an untwisted dsDNA by a nucleoprotein filament leads to an exchanged duplex that remains topologically linked to the exchanged single strand , suggesting multiple initiations of strand exchange on the same molecule .
	manualset3
104237	6	401551	13	NULL	NULL	0	NULL	molecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Invasion of an untwisted dsDNA by a nucleoprotein filament leads to an exchanged duplex that remains topologically linked to the exchanged single strand , suggesting multiple initiations of strand exchange on the same molecule .
	manualset3
108301	7	401551	13	NULL	NULL	0	NULL	exchanged duplex	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Invasion of an untwisted dsDNA by a nucleoprotein filament leads to an exchanged duplex that remains topologically linked to the exchanged single strand , suggesting multiple initiations of strand exchange on the same molecule .
	manualset3
104238	1	401552	13	NULL	NULL	0	NULL	Invasive alien species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Invasive alien species are among the primary causes of biodiversity change globally , with the risks thereof broadly understood for most regions of the world .
	manualset3
104239	2	401552	13	NULL	NULL	NULL	NULL	primary causes	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Invasive alien species are among the primary causes of biodiversity change globally , with the risks thereof broadly understood for most regions of the world .
	manualset3
104240	3	401552	13	NULL	NULL	0	NULL	biodiversity change globally	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Invasive alien species are among the primary causes of biodiversity change globally , with the risks thereof broadly understood for most regions of the world .
	manualset3
104241	4	401552	13	NULL	NULL	0	NULL	risks 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Invasive alien species are among the primary causes of biodiversity change globally , with the risks thereof broadly understood for most regions of the world .
	manualset3
104242	5	401552	13	NULL	NULL	0	NULL	most regions	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Invasive alien species are among the primary causes of biodiversity change globally , with the risks thereof broadly understood for most regions of the world .
	manualset3
104243	6	401552	13	NULL	NULL	0	NULL	world	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Invasive alien species are among the primary causes of biodiversity change globally , with the risks thereof broadly understood for most regions of the world .
	manualset3
104253	1	401553	13	NULL	NULL	0	NULL	Invasive techniques	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Invasive and noninvasive techniques in the detection and evaluation of acute venous thrombosis .
	manualset3
104255	2	401553	13	NULL	NULL	0	NULL	noninvasive techniques	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Invasive and noninvasive techniques in the detection and evaluation of acute venous thrombosis .
	manualset3
104259	3	401553	13	NULL	NULL	0	NULL	detection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Invasive and noninvasive techniques in the detection and evaluation of acute venous thrombosis .
	manualset3
104261	4	401553	13	NULL	NULL	0	NULL	evaluation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Invasive and noninvasive techniques in the detection and evaluation of acute venous thrombosis .
	manualset3
104262	5	401553	13	NULL	NULL	0	NULL	acute venous thrombosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Invasive and noninvasive techniques in the detection and evaluation of acute venous thrombosis .
	manualset3
104270	1	401554	13	NULL	NULL	0	NULL	Invasive aspergillosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Invasive aspergillosis is an emerging infection mainly affecting immunocompromised patients .
	manualset3
104271	2	401554	13	NULL	NULL	0	NULL	infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Invasive aspergillosis is an emerging infection mainly affecting immunocompromised patients .
	manualset3
104272	3	401554	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Invasive aspergillosis is an emerging infection mainly affecting immunocompromised patients .
	manualset3
104320	1	401555	13	NULL	NULL	0	NULL	Invasive ductal carcinoma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Invasive ductal carcinoma of the pancreas was resected in 121 patients in our institution from 1992 through 2005 .
	manualset3
104321	2	401555	13	NULL	NULL	0	NULL	 pancreas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Invasive ductal carcinoma of the pancreas was resected in 121 patients in our institution from 1992 through 2005 .
	manualset3
104322	3	401555	13	NULL	NULL	0	NULL	121 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Invasive ductal carcinoma of the pancreas was resected in 121 patients in our institution from 1992 through 2005 .
	manualset3
104323	4	401555	13	NULL	NULL	0	NULL	institution	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Invasive ductal carcinoma of the pancreas was resected in 121 patients in our institution from 1992 through 2005 .
	manualset3
104324	5	401555	13	NULL	NULL	0	NULL	1992	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Invasive ductal carcinoma of the pancreas was resected in 121 patients in our institution from 1992 through 2005 .
	manualset3
104325	6	401555	13	NULL	NULL	0	NULL	 2005	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Invasive ductal carcinoma of the pancreas was resected in 121 patients in our institution from 1992 through 2005 .
	manualset3
104326	1	401556	13	NULL	NULL	0	NULL	Assorption 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Assorption of strontium-90 by krill ) .
	manualset3
104327	2	401556	13	NULL	NULL	0	NULL	strontium-90	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Assorption of strontium-90 by krill ) .
	manualset3
104328	3	401556	13	NULL	NULL	0	NULL	krill 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Assorption of strontium-90 by krill ) .
	manualset3
104335	1	401557	13	NULL	NULL	0	NULL	4 study sites	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	4 study sites were selected from each patient which had pocket depths greater than 4 mm and bleeding upon probing .
	manualset3
104336	2	401557	13	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	4 study sites were selected from each patient which had pocket depths greater than 4 mm and bleeding upon probing .
	manualset3
104337	3	401557	13	NULL	NULL	0	NULL	 pocket depths	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	4 study sites were selected from each patient which had pocket depths greater than 4 mm and bleeding upon probing .
	manualset3
104338	4	401557	13	NULL	NULL	0	NULL	greater than 4 mm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	4 study sites were selected from each patient which had pocket depths greater than 4 mm and bleeding upon probing .
	manualset3
104346	5	401557	13	NULL	NULL	0	NULL	bleeding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	4 study sites were selected from each patient which had pocket depths greater than 4 mm and bleeding upon probing .
	manualset3
104348	1	401558	13	NULL	NULL	0	NULL	Inverted papilloma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inverted papilloma of the nose and paranasal sinuses : a study of 56 cases and review of the literature .
	manualset3
104349	2	401558	13	NULL	NULL	0	NULL	nose	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Inverted papilloma of the nose and paranasal sinuses : a study of 56 cases and review of the literature .
	manualset3
104350	3	401558	13	NULL	NULL	0	NULL	paranasal sinuses	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Inverted papilloma of the nose and paranasal sinuses : a study of 56 cases and review of the literature .
	manualset3
104351	4	401558	13	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Inverted papilloma of the nose and paranasal sinuses : a study of 56 cases and review of the literature .
	manualset3
104352	5	401558	13	NULL	NULL	0	NULL	56 cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Inverted papilloma of the nose and paranasal sinuses : a study of 56 cases and review of the literature .
	manualset3
104353	6	401558	13	NULL	NULL	0	NULL	review	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inverted papilloma of the nose and paranasal sinuses : a study of 56 cases and review of the literature .
	manualset3
104354	7	401558	13	NULL	NULL	0	NULL	literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Inverted papilloma of the nose and paranasal sinuses : a study of 56 cases and review of the literature .
	manualset3
104381	1	401559	13	NULL	NULL	NULL	NULL	frequency 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Investigating one frequency ( 7 Hz ) , we found two discrete periods of sensitivity to vibration ; during the first period , vibration affected the same LR pathway as nocodazole , while during the second period , vibration affected the integrity of the epithelial barrier ; both are required for normal LR patterning .
	manualset3
104386	2	401559	13	NULL	NULL	0	NULL	7 Hz	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigating one frequency ( 7 Hz ) , we found two discrete periods of sensitivity to vibration ; during the first period , vibration affected the same LR pathway as nocodazole , while during the second period , vibration affected the integrity of the epithelial barrier ; both are required for normal LR patterning .
	manualset3
104387	3	401559	13	NULL	NULL	0	NULL	sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigating one frequency ( 7 Hz ) , we found two discrete periods of sensitivity to vibration ; during the first period , vibration affected the same LR pathway as nocodazole , while during the second period , vibration affected the integrity of the epithelial barrier ; both are required for normal LR patterning .
	manualset3
104388	4	401559	13	NULL	NULL	0	NULL	vibration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigating one frequency ( 7 Hz ) , we found two discrete periods of sensitivity to vibration ; during the first period , vibration affected the same LR pathway as nocodazole , while during the second period , vibration affected the integrity of the epithelial barrier ; both are required for normal LR patterning .
	manualset3
104389	5	401559	13	NULL	NULL	0	NULL	first period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigating one frequency ( 7 Hz ) , we found two discrete periods of sensitivity to vibration ; during the first period , vibration affected the same LR pathway as nocodazole , while during the second period , vibration affected the integrity of the epithelial barrier ; both are required for normal LR patterning .
	manualset3
104391	6	401559	13	NULL	NULL	0	NULL	vibration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigating one frequency ( 7 Hz ) , we found two discrete periods of sensitivity to vibration ; during the first period , vibration affected the same LR pathway as nocodazole , while during the second period , vibration affected the integrity of the epithelial barrier ; both are required for normal LR patterning .
	manualset3
104393	7	401559	13	NULL	NULL	0	NULL	LR pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigating one frequency ( 7 Hz ) , we found two discrete periods of sensitivity to vibration ; during the first period , vibration affected the same LR pathway as nocodazole , while during the second period , vibration affected the integrity of the epithelial barrier ; both are required for normal LR patterning .
	manualset3
104398	8	401559	13	NULL	NULL	0	NULL	nocodazole 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigating one frequency ( 7 Hz ) , we found two discrete periods of sensitivity to vibration ; during the first period , vibration affected the same LR pathway as nocodazole , while during the second period , vibration affected the integrity of the epithelial barrier ; both are required for normal LR patterning .
	manualset3
104399	9	401559	13	NULL	NULL	0	NULL	second period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigating one frequency ( 7 Hz ) , we found two discrete periods of sensitivity to vibration ; during the first period , vibration affected the same LR pathway as nocodazole , while during the second period , vibration affected the integrity of the epithelial barrier ; both are required for normal LR patterning .
	manualset3
104400	10	401559	13	NULL	NULL	0	NULL	vibration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigating one frequency ( 7 Hz ) , we found two discrete periods of sensitivity to vibration ; during the first period , vibration affected the same LR pathway as nocodazole , while during the second period , vibration affected the integrity of the epithelial barrier ; both are required for normal LR patterning .
	manualset3
104417	11	401559	13	NULL	NULL	0	NULL	integrity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigating one frequency ( 7 Hz ) , we found two discrete periods of sensitivity to vibration ; during the first period , vibration affected the same LR pathway as nocodazole , while during the second period , vibration affected the integrity of the epithelial barrier ; both are required for normal LR patterning .
	manualset3
104422	12	401559	13	NULL	NULL	0	NULL	epithelial barrier	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigating one frequency ( 7 Hz ) , we found two discrete periods of sensitivity to vibration ; during the first period , vibration affected the same LR pathway as nocodazole , while during the second period , vibration affected the integrity of the epithelial barrier ; both are required for normal LR patterning .
	manualset3
104425	13	401559	13	NULL	NULL	0	NULL	LR patterning 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigating one frequency ( 7 Hz ) , we found two discrete periods of sensitivity to vibration ; during the first period , vibration affected the same LR pathway as nocodazole , while during the second period , vibration affected the integrity of the epithelial barrier ; both are required for normal LR patterning .
	manualset3
108302	14	401559	13	NULL	NULL	0	NULL	two discrete periods	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigating one frequency ( 7 Hz ) , we found two discrete periods of sensitivity to vibration ; during the first period , vibration affected the same LR pathway as nocodazole , while during the second period , vibration affected the integrity of the epithelial barrier ; both are required for normal LR patterning .
	manualset3
104434	1	401560	13	NULL	NULL	0	NULL	Investigation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of influenza viruses isolated from man and animals and having hemagglutinin of the H3 subtype according to the new nomenclature ( H3 , Heq2 and Hav7 according to the old nomenclature ) by serological methods ( including the use of monoclonal antibody ) and oligopeptide mapping showed that many animal isolates reflected an antigenic drift of the Hong Kong virus series which has been going on since 1968 until now .
	manualset3
104435	2	401560	13	NULL	NULL	0	NULL	influenza viruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of influenza viruses isolated from man and animals and having hemagglutinin of the H3 subtype according to the new nomenclature ( H3 , Heq2 and Hav7 according to the old nomenclature ) by serological methods ( including the use of monoclonal antibody ) and oligopeptide mapping showed that many animal isolates reflected an antigenic drift of the Hong Kong virus series which has been going on since 1968 until now .
	manualset3
104436	3	401560	13	NULL	NULL	0	NULL	man	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of influenza viruses isolated from man and animals and having hemagglutinin of the H3 subtype according to the new nomenclature ( H3 , Heq2 and Hav7 according to the old nomenclature ) by serological methods ( including the use of monoclonal antibody ) and oligopeptide mapping showed that many animal isolates reflected an antigenic drift of the Hong Kong virus series which has been going on since 1968 until now .
	manualset3
104437	4	401560	13	NULL	NULL	0	NULL	animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of influenza viruses isolated from man and animals and having hemagglutinin of the H3 subtype according to the new nomenclature ( H3 , Heq2 and Hav7 according to the old nomenclature ) by serological methods ( including the use of monoclonal antibody ) and oligopeptide mapping showed that many animal isolates reflected an antigenic drift of the Hong Kong virus series which has been going on since 1968 until now .
	manualset3
104446	5	401560	13	NULL	NULL	NULL	NULL	hemagglutinin of the H3 subtype	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Investigation of influenza viruses isolated from man and animals and having hemagglutinin of the H3 subtype according to the new nomenclature ( H3 , Heq2 and Hav7 according to the old nomenclature ) by serological methods ( including the use of monoclonal antibody ) and oligopeptide mapping showed that many animal isolates reflected an antigenic drift of the Hong Kong virus series which has been going on since 1968 until now .
	manualset3
104447	6	401560	13	NULL	NULL	NULL	NULL	new nomenclature	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Investigation of influenza viruses isolated from man and animals and having hemagglutinin of the H3 subtype according to the new nomenclature ( H3 , Heq2 and Hav7 according to the old nomenclature ) by serological methods ( including the use of monoclonal antibody ) and oligopeptide mapping showed that many animal isolates reflected an antigenic drift of the Hong Kong virus series which has been going on since 1968 until now .
	manualset3
104448	7	401560	13	NULL	NULL	0	NULL	H3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of influenza viruses isolated from man and animals and having hemagglutinin of the H3 subtype according to the new nomenclature ( H3 , Heq2 and Hav7 according to the old nomenclature ) by serological methods ( including the use of monoclonal antibody ) and oligopeptide mapping showed that many animal isolates reflected an antigenic drift of the Hong Kong virus series which has been going on since 1968 until now .
	manualset3
104449	8	401560	13	NULL	NULL	0	NULL	Heq2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of influenza viruses isolated from man and animals and having hemagglutinin of the H3 subtype according to the new nomenclature ( H3 , Heq2 and Hav7 according to the old nomenclature ) by serological methods ( including the use of monoclonal antibody ) and oligopeptide mapping showed that many animal isolates reflected an antigenic drift of the Hong Kong virus series which has been going on since 1968 until now .
	manualset3
104450	9	401560	13	NULL	NULL	0	NULL	Hav7 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of influenza viruses isolated from man and animals and having hemagglutinin of the H3 subtype according to the new nomenclature ( H3 , Heq2 and Hav7 according to the old nomenclature ) by serological methods ( including the use of monoclonal antibody ) and oligopeptide mapping showed that many animal isolates reflected an antigenic drift of the Hong Kong virus series which has been going on since 1968 until now .
	manualset3
104452	10	401560	13	NULL	NULL	0	NULL	 old nomenclature 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of influenza viruses isolated from man and animals and having hemagglutinin of the H3 subtype according to the new nomenclature ( H3 , Heq2 and Hav7 according to the old nomenclature ) by serological methods ( including the use of monoclonal antibody ) and oligopeptide mapping showed that many animal isolates reflected an antigenic drift of the Hong Kong virus series which has been going on since 1968 until now .
	manualset3
104453	11	401560	13	NULL	NULL	0	NULL	serological methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of influenza viruses isolated from man and animals and having hemagglutinin of the H3 subtype according to the new nomenclature ( H3 , Heq2 and Hav7 according to the old nomenclature ) by serological methods ( including the use of monoclonal antibody ) and oligopeptide mapping showed that many animal isolates reflected an antigenic drift of the Hong Kong virus series which has been going on since 1968 until now .
	manualset3
104454	12	401560	13	NULL	NULL	0	NULL	use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of influenza viruses isolated from man and animals and having hemagglutinin of the H3 subtype according to the new nomenclature ( H3 , Heq2 and Hav7 according to the old nomenclature ) by serological methods ( including the use of monoclonal antibody ) and oligopeptide mapping showed that many animal isolates reflected an antigenic drift of the Hong Kong virus series which has been going on since 1968 until now .
	manualset3
104455	13	401560	13	NULL	NULL	0	NULL	monoclonal antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of influenza viruses isolated from man and animals and having hemagglutinin of the H3 subtype according to the new nomenclature ( H3 , Heq2 and Hav7 according to the old nomenclature ) by serological methods ( including the use of monoclonal antibody ) and oligopeptide mapping showed that many animal isolates reflected an antigenic drift of the Hong Kong virus series which has been going on since 1968 until now .
	manualset3
104456	14	401560	13	NULL	NULL	0	NULL	oligopeptide mapping	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of influenza viruses isolated from man and animals and having hemagglutinin of the H3 subtype according to the new nomenclature ( H3 , Heq2 and Hav7 according to the old nomenclature ) by serological methods ( including the use of monoclonal antibody ) and oligopeptide mapping showed that many animal isolates reflected an antigenic drift of the Hong Kong virus series which has been going on since 1968 until now .
	manualset3
104457	15	401560	13	NULL	NULL	0	NULL	animal isolates 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of influenza viruses isolated from man and animals and having hemagglutinin of the H3 subtype according to the new nomenclature ( H3 , Heq2 and Hav7 according to the old nomenclature ) by serological methods ( including the use of monoclonal antibody ) and oligopeptide mapping showed that many animal isolates reflected an antigenic drift of the Hong Kong virus series which has been going on since 1968 until now .
	manualset3
104458	16	401560	13	NULL	NULL	0	NULL	antigenic drift 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of influenza viruses isolated from man and animals and having hemagglutinin of the H3 subtype according to the new nomenclature ( H3 , Heq2 and Hav7 according to the old nomenclature ) by serological methods ( including the use of monoclonal antibody ) and oligopeptide mapping showed that many animal isolates reflected an antigenic drift of the Hong Kong virus series which has been going on since 1968 until now .
	manualset3
104459	17	401560	13	NULL	NULL	0	NULL	Hong Kong virus series	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of influenza viruses isolated from man and animals and having hemagglutinin of the H3 subtype according to the new nomenclature ( H3 , Heq2 and Hav7 according to the old nomenclature ) by serological methods ( including the use of monoclonal antibody ) and oligopeptide mapping showed that many animal isolates reflected an antigenic drift of the Hong Kong virus series which has been going on since 1968 until now .
	manualset3
104461	18	401560	13	NULL	NULL	0	NULL	1968	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of influenza viruses isolated from man and animals and having hemagglutinin of the H3 subtype according to the new nomenclature ( H3 , Heq2 and Hav7 according to the old nomenclature ) by serological methods ( including the use of monoclonal antibody ) and oligopeptide mapping showed that many animal isolates reflected an antigenic drift of the Hong Kong virus series which has been going on since 1968 until now .
	manualset3
104462	1	401561	13	NULL	NULL	0	NULL	Investigation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of intensity thresholds for ultrasound tissue erosion .
	manualset3
104465	2	401561	13	NULL	NULL	0	NULL	intensity thresholds 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of intensity thresholds for ultrasound tissue erosion .
	manualset3
104467	3	401561	13	NULL	NULL	0	NULL	ultrasound tissue erosion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of intensity thresholds for ultrasound tissue erosion .
	manualset3
104469	1	401562	13	NULL	NULL	NULL	NULL	Investigation 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Investigation of nicotine binding to THP-1 cells : evidence for a non-cholinergic binding site .
	manualset3
104470	2	401562	13	NULL	NULL	0	NULL	nicotine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of nicotine binding to THP-1 cells : evidence for a non-cholinergic binding site .
	manualset3
104471	3	401562	13	NULL	NULL	0	NULL	binding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of nicotine binding to THP-1 cells : evidence for a non-cholinergic binding site .
	manualset3
104472	4	401562	13	NULL	NULL	0	NULL	THP-1 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of nicotine binding to THP-1 cells : evidence for a non-cholinergic binding site .
	manualset3
104474	5	401562	13	NULL	NULL	NULL	NULL	evidence	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Investigation of nicotine binding to THP-1 cells : evidence for a non-cholinergic binding site .
	manualset3
108304	6	401562	13	NULL	NULL	0	NULL	non-cholinergic binding site	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of nicotine binding to THP-1 cells : evidence for a non-cholinergic binding site .
	manualset3
104622	1	401563	13	NULL	NULL	0	NULL	Investigation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of other clinically distinct syndromes associated with lipomatosis and overgrowth has established germline and germline mosaic PTEN mutations in several patients with Proteus syndrome .
	manualset3
104623	2	401563	13	NULL	NULL	0	NULL	clinically distinct syndromes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of other clinically distinct syndromes associated with lipomatosis and overgrowth has established germline and germline mosaic PTEN mutations in several patients with Proteus syndrome .
	manualset3
104624	3	401563	13	NULL	NULL	0	NULL	lipomatosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of other clinically distinct syndromes associated with lipomatosis and overgrowth has established germline and germline mosaic PTEN mutations in several patients with Proteus syndrome .
	manualset3
104625	4	401563	13	NULL	NULL	0	NULL	overgrowth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of other clinically distinct syndromes associated with lipomatosis and overgrowth has established germline and germline mosaic PTEN mutations in several patients with Proteus syndrome .
	manualset3
104626	5	401563	13	NULL	NULL	0	NULL	germline mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of other clinically distinct syndromes associated with lipomatosis and overgrowth has established germline and germline mosaic PTEN mutations in several patients with Proteus syndrome .
	manualset3
104627	6	401563	13	NULL	NULL	0	NULL	germline mosaic PTEN mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of other clinically distinct syndromes associated with lipomatosis and overgrowth has established germline and germline mosaic PTEN mutations in several patients with Proteus syndrome .
	manualset3
104628	7	401563	13	NULL	NULL	0	NULL	several patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of other clinically distinct syndromes associated with lipomatosis and overgrowth has established germline and germline mosaic PTEN mutations in several patients with Proteus syndrome .
	manualset3
104629	8	401563	13	NULL	NULL	0	NULL	Proteus syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of other clinically distinct syndromes associated with lipomatosis and overgrowth has established germline and germline mosaic PTEN mutations in several patients with Proteus syndrome .
	manualset3
104630	1	401564	13	NULL	NULL	0	NULL	Investigation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of the Li + transport mechanism revealed that contribution from the Li + diffusion together with its coordination shell to the total Li + transport is similar to the contribution arising from Li + exchanging solvent molecules in its first coordination shell with solvents from the outer shells .
	manualset3
104631	2	401564	13	NULL	NULL	0	NULL	Li + transport mechanism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of the Li + transport mechanism revealed that contribution from the Li + diffusion together with its coordination shell to the total Li + transport is similar to the contribution arising from Li + exchanging solvent molecules in its first coordination shell with solvents from the outer shells .
	manualset3
104632	3	401564	13	NULL	NULL	0	NULL	contribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of the Li + transport mechanism revealed that contribution from the Li + diffusion together with its coordination shell to the total Li + transport is similar to the contribution arising from Li + exchanging solvent molecules in its first coordination shell with solvents from the outer shells .
	manualset3
104633	4	401564	13	NULL	NULL	0	NULL	Li + diffusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of the Li + transport mechanism revealed that contribution from the Li + diffusion together with its coordination shell to the total Li + transport is similar to the contribution arising from Li + exchanging solvent molecules in its first coordination shell with solvents from the outer shells .
	manualset3
104634	5	401564	13	NULL	NULL	0	NULL	coordination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of the Li + transport mechanism revealed that contribution from the Li + diffusion together with its coordination shell to the total Li + transport is similar to the contribution arising from Li + exchanging solvent molecules in its first coordination shell with solvents from the outer shells .
	manualset3
104635	6	401564	13	NULL	NULL	0	NULL	shell 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of the Li + transport mechanism revealed that contribution from the Li + diffusion together with its coordination shell to the total Li + transport is similar to the contribution arising from Li + exchanging solvent molecules in its first coordination shell with solvents from the outer shells .
	manualset3
104636	7	401564	13	NULL	NULL	0	NULL	 total Li + transport 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of the Li + transport mechanism revealed that contribution from the Li + diffusion together with its coordination shell to the total Li + transport is similar to the contribution arising from Li + exchanging solvent molecules in its first coordination shell with solvents from the outer shells .
	manualset3
104637	8	401564	13	NULL	NULL	0	NULL	contribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of the Li + transport mechanism revealed that contribution from the Li + diffusion together with its coordination shell to the total Li + transport is similar to the contribution arising from Li + exchanging solvent molecules in its first coordination shell with solvents from the outer shells .
	manualset3
104638	9	401564	13	NULL	NULL	0	NULL	Li + exchanging solvent molecules	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of the Li + transport mechanism revealed that contribution from the Li + diffusion together with its coordination shell to the total Li + transport is similar to the contribution arising from Li + exchanging solvent molecules in its first coordination shell with solvents from the outer shells .
	manualset3
104639	10	401564	13	NULL	NULL	0	NULL	coordination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of the Li + transport mechanism revealed that contribution from the Li + diffusion together with its coordination shell to the total Li + transport is similar to the contribution arising from Li + exchanging solvent molecules in its first coordination shell with solvents from the outer shells .
	manualset3
104640	11	401564	13	NULL	NULL	0	NULL	shell	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of the Li + transport mechanism revealed that contribution from the Li + diffusion together with its coordination shell to the total Li + transport is similar to the contribution arising from Li + exchanging solvent molecules in its first coordination shell with solvents from the outer shells .
	manualset3
104641	12	401564	13	NULL	NULL	0	NULL	solvents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of the Li + transport mechanism revealed that contribution from the Li + diffusion together with its coordination shell to the total Li + transport is similar to the contribution arising from Li + exchanging solvent molecules in its first coordination shell with solvents from the outer shells .
	manualset3
104642	13	401564	13	NULL	NULL	0	NULL	shells	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of the Li + transport mechanism revealed that contribution from the Li + diffusion together with its coordination shell to the total Li + transport is similar to the contribution arising from Li + exchanging solvent molecules in its first coordination shell with solvents from the outer shells .
	manualset3
104643	1	401565	13	NULL	NULL	0	NULL	Investigation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of the radical chemistry of the three salts using pulse radiolysis indicated that oxidation of NaMeS ( 2 ) O ( 2 ) H ( 2 ) O involves formation of a sulfur-centred radical rather than hydrogen abstraction from the methyl substituent , whereas oxidation of the aromatic ring is the preferred pathway for the phenyl and p-tolyl derivatives .
	manualset3
104644	2	401565	13	NULL	NULL	0	NULL	radical chemistry 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of the radical chemistry of the three salts using pulse radiolysis indicated that oxidation of NaMeS ( 2 ) O ( 2 ) H ( 2 ) O involves formation of a sulfur-centred radical rather than hydrogen abstraction from the methyl substituent , whereas oxidation of the aromatic ring is the preferred pathway for the phenyl and p-tolyl derivatives .
	manualset3
104645	3	401565	13	NULL	NULL	0	NULL	 three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of the radical chemistry of the three salts using pulse radiolysis indicated that oxidation of NaMeS ( 2 ) O ( 2 ) H ( 2 ) O involves formation of a sulfur-centred radical rather than hydrogen abstraction from the methyl substituent , whereas oxidation of the aromatic ring is the preferred pathway for the phenyl and p-tolyl derivatives .
	manualset3
104646	4	401565	13	NULL	NULL	0	NULL	salts 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of the radical chemistry of the three salts using pulse radiolysis indicated that oxidation of NaMeS ( 2 ) O ( 2 ) H ( 2 ) O involves formation of a sulfur-centred radical rather than hydrogen abstraction from the methyl substituent , whereas oxidation of the aromatic ring is the preferred pathway for the phenyl and p-tolyl derivatives .
	manualset3
104647	5	401565	13	NULL	NULL	0	NULL	pulse radiolysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of the radical chemistry of the three salts using pulse radiolysis indicated that oxidation of NaMeS ( 2 ) O ( 2 ) H ( 2 ) O involves formation of a sulfur-centred radical rather than hydrogen abstraction from the methyl substituent , whereas oxidation of the aromatic ring is the preferred pathway for the phenyl and p-tolyl derivatives .
	manualset3
104648	6	401565	13	NULL	NULL	0	NULL	oxidation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of the radical chemistry of the three salts using pulse radiolysis indicated that oxidation of NaMeS ( 2 ) O ( 2 ) H ( 2 ) O involves formation of a sulfur-centred radical rather than hydrogen abstraction from the methyl substituent , whereas oxidation of the aromatic ring is the preferred pathway for the phenyl and p-tolyl derivatives .
	manualset3
104649	7	401565	13	NULL	NULL	0	NULL	NaMeS ( 2 ) O ( 2 ) H ( 2 ) O	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of the radical chemistry of the three salts using pulse radiolysis indicated that oxidation of NaMeS ( 2 ) O ( 2 ) H ( 2 ) O involves formation of a sulfur-centred radical rather than hydrogen abstraction from the methyl substituent , whereas oxidation of the aromatic ring is the preferred pathway for the phenyl and p-tolyl derivatives .
	manualset3
104650	8	401565	13	NULL	NULL	0	NULL	formation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of the radical chemistry of the three salts using pulse radiolysis indicated that oxidation of NaMeS ( 2 ) O ( 2 ) H ( 2 ) O involves formation of a sulfur-centred radical rather than hydrogen abstraction from the methyl substituent , whereas oxidation of the aromatic ring is the preferred pathway for the phenyl and p-tolyl derivatives .
	manualset3
104651	10	401565	13	NULL	NULL	NULL	NULL	hydrogen	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Investigation of the radical chemistry of the three salts using pulse radiolysis indicated that oxidation of NaMeS ( 2 ) O ( 2 ) H ( 2 ) O involves formation of a sulfur-centred radical rather than hydrogen abstraction from the methyl substituent , whereas oxidation of the aromatic ring is the preferred pathway for the phenyl and p-tolyl derivatives .
	manualset3
104652	9	401565	13	NULL	NULL	0	NULL	sulfur-centred radical	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of the radical chemistry of the three salts using pulse radiolysis indicated that oxidation of NaMeS ( 2 ) O ( 2 ) H ( 2 ) O involves formation of a sulfur-centred radical rather than hydrogen abstraction from the methyl substituent , whereas oxidation of the aromatic ring is the preferred pathway for the phenyl and p-tolyl derivatives .
	manualset3
104653	11	401565	13	NULL	NULL	0	NULL	abstraction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of the radical chemistry of the three salts using pulse radiolysis indicated that oxidation of NaMeS ( 2 ) O ( 2 ) H ( 2 ) O involves formation of a sulfur-centred radical rather than hydrogen abstraction from the methyl substituent , whereas oxidation of the aromatic ring is the preferred pathway for the phenyl and p-tolyl derivatives .
	manualset3
104654	12	401565	13	NULL	NULL	0	NULL	methyl substituent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of the radical chemistry of the three salts using pulse radiolysis indicated that oxidation of NaMeS ( 2 ) O ( 2 ) H ( 2 ) O involves formation of a sulfur-centred radical rather than hydrogen abstraction from the methyl substituent , whereas oxidation of the aromatic ring is the preferred pathway for the phenyl and p-tolyl derivatives .
	manualset3
104655	13	401565	13	NULL	NULL	0	NULL	oxidation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of the radical chemistry of the three salts using pulse radiolysis indicated that oxidation of NaMeS ( 2 ) O ( 2 ) H ( 2 ) O involves formation of a sulfur-centred radical rather than hydrogen abstraction from the methyl substituent , whereas oxidation of the aromatic ring is the preferred pathway for the phenyl and p-tolyl derivatives .
	manualset3
104656	14	401565	13	NULL	NULL	0	NULL	aromatic ring	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of the radical chemistry of the three salts using pulse radiolysis indicated that oxidation of NaMeS ( 2 ) O ( 2 ) H ( 2 ) O involves formation of a sulfur-centred radical rather than hydrogen abstraction from the methyl substituent , whereas oxidation of the aromatic ring is the preferred pathway for the phenyl and p-tolyl derivatives .
	manualset3
104657	15	401565	13	NULL	NULL	0	NULL	 pathway	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of the radical chemistry of the three salts using pulse radiolysis indicated that oxidation of NaMeS ( 2 ) O ( 2 ) H ( 2 ) O involves formation of a sulfur-centred radical rather than hydrogen abstraction from the methyl substituent , whereas oxidation of the aromatic ring is the preferred pathway for the phenyl and p-tolyl derivatives .
	manualset3
104658	16	401565	13	NULL	NULL	0	NULL	phenyl derivatives	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of the radical chemistry of the three salts using pulse radiolysis indicated that oxidation of NaMeS ( 2 ) O ( 2 ) H ( 2 ) O involves formation of a sulfur-centred radical rather than hydrogen abstraction from the methyl substituent , whereas oxidation of the aromatic ring is the preferred pathway for the phenyl and p-tolyl derivatives .
	manualset3
104659	17	401565	13	NULL	NULL	0	NULL	p-tolyl derivatives	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of the radical chemistry of the three salts using pulse radiolysis indicated that oxidation of NaMeS ( 2 ) O ( 2 ) H ( 2 ) O involves formation of a sulfur-centred radical rather than hydrogen abstraction from the methyl substituent , whereas oxidation of the aromatic ring is the preferred pathway for the phenyl and p-tolyl derivatives .
	manualset3
104660	1	401566	13	NULL	NULL	0	NULL	Investigation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation on the mechanisms of the failure of human influenza virus to replicate in chick embryo cell cultures .
	manualset3
104661	2	401566	13	NULL	NULL	0	NULL	mechanisms of the failure 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation on the mechanisms of the failure of human influenza virus to replicate in chick embryo cell cultures .
	manualset3
104662	3	401566	13	NULL	NULL	0	NULL	human influenza virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation on the mechanisms of the failure of human influenza virus to replicate in chick embryo cell cultures .
	manualset3
104663	4	401566	13	NULL	NULL	0	NULL	chick embryo cell cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation on the mechanisms of the failure of human influenza virus to replicate in chick embryo cell cultures .
	manualset3
104664	1	401567	13	NULL	NULL	0	NULL	Investigations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigations of factors that influence the acrylamide content of heated foodstuffs .
	manualset3
104665	2	401567	13	NULL	NULL	0	NULL	factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigations of factors that influence the acrylamide content of heated foodstuffs .
	manualset3
104666	3	401567	13	NULL	NULL	0	NULL	influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigations of factors that influence the acrylamide content of heated foodstuffs .
	manualset3
104667	4	401567	13	NULL	NULL	0	NULL	 acrylamide content 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigations of factors that influence the acrylamide content of heated foodstuffs .
	manualset3
104668	5	401567	13	NULL	NULL	0	NULL	foodstuffs	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigations of factors that influence the acrylamide content of heated foodstuffs .
	manualset3
104669	1	401568	13	NULL	NULL	0	NULL	Investigations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigations of families with an apparent hereditary cancer and constitutional chromosome rearrangements have led to the molecular identification of tumor suppressor genes .
	manualset3
104670	2	401568	13	NULL	NULL	0	NULL	families	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigations of families with an apparent hereditary cancer and constitutional chromosome rearrangements have led to the molecular identification of tumor suppressor genes .
	manualset3
104671	3	401568	13	NULL	NULL	0	NULL	hereditary cancer 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigations of families with an apparent hereditary cancer and constitutional chromosome rearrangements have led to the molecular identification of tumor suppressor genes .
	manualset3
104672	4	401568	13	NULL	NULL	0	NULL	constitutional chromosome rearrangements	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigations of families with an apparent hereditary cancer and constitutional chromosome rearrangements have led to the molecular identification of tumor suppressor genes .
	manualset3
104673	5	401568	13	NULL	NULL	0	NULL	molecular identification	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigations of families with an apparent hereditary cancer and constitutional chromosome rearrangements have led to the molecular identification of tumor suppressor genes .
	manualset3
104674	6	401568	13	NULL	NULL	0	NULL	tumor suppressor genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigations of families with an apparent hereditary cancer and constitutional chromosome rearrangements have led to the molecular identification of tumor suppressor genes .
	manualset3
104675	1	401569	13	NULL	NULL	0	NULL	Investigations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigations revealed a raised acute phase response ( C reactive protein 97 mg/l , erythrocyte sedimentation rate ) 100 mm/h ) , leucocytosis and thrombocytosis .
	manualset3
104676	2	401569	13	NULL	NULL	0	NULL	acute phase response 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigations revealed a raised acute phase response ( C reactive protein 97 mg/l , erythrocyte sedimentation rate ) 100 mm/h ) , leucocytosis and thrombocytosis .
	manualset3
104677	3	401569	13	NULL	NULL	0	NULL	C reactive protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigations revealed a raised acute phase response ( C reactive protein 97 mg/l , erythrocyte sedimentation rate ) 100 mm/h ) , leucocytosis and thrombocytosis .
	manualset3
104678	4	401569	13	NULL	NULL	0	NULL	97 mg/l	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigations revealed a raised acute phase response ( C reactive protein 97 mg/l , erythrocyte sedimentation rate ) 100 mm/h ) , leucocytosis and thrombocytosis .
	manualset3
104679	5	401569	13	NULL	NULL	NULL	NULL	erythrocyte sedimentation rate	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Investigations revealed a raised acute phase response ( C reactive protein 97 mg/l , erythrocyte sedimentation rate ) 100 mm/h ) , leucocytosis and thrombocytosis .
	manualset3
104680	6	401569	13	NULL	NULL	0	NULL	100 mm/h 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigations revealed a raised acute phase response ( C reactive protein 97 mg/l , erythrocyte sedimentation rate ) 100 mm/h ) , leucocytosis and thrombocytosis .
	manualset3
104681	7	401569	13	NULL	NULL	0	NULL	leucocytosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigations revealed a raised acute phase response ( C reactive protein 97 mg/l , erythrocyte sedimentation rate ) 100 mm/h ) , leucocytosis and thrombocytosis .
	manualset3
104682	8	401569	13	NULL	NULL	0	NULL	 thrombocytosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigations revealed a raised acute phase response ( C reactive protein 97 mg/l , erythrocyte sedimentation rate ) 100 mm/h ) , leucocytosis and thrombocytosis .
	manualset3
104683	1	401570	13	NULL	NULL	0	NULL	Investigators 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigators are searching for HLA-DR4 containing chromosomes in IDDM which show similar patterns of restriction enzyme polymorphism .
	manualset3
104684	2	401570	13	NULL	NULL	0	NULL	HLA-DR4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigators are searching for HLA-DR4 containing chromosomes in IDDM which show similar patterns of restriction enzyme polymorphism .
	manualset3
104685	3	401570	13	NULL	NULL	0	NULL	chromosomes 	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigators are searching for HLA-DR4 containing chromosomes in IDDM which show similar patterns of restriction enzyme polymorphism .
	manualset3
104686	4	401570	13	NULL	NULL	0	NULL	IDDM	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigators are searching for HLA-DR4 containing chromosomes in IDDM which show similar patterns of restriction enzyme polymorphism .
	manualset3
104687	5	401570	13	NULL	NULL	0	NULL	similar patterns	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigators are searching for HLA-DR4 containing chromosomes in IDDM which show similar patterns of restriction enzyme polymorphism .
	manualset3
104688	6	401570	13	NULL	NULL	0	NULL	restriction enzyme polymorphism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigators are searching for HLA-DR4 containing chromosomes in IDDM which show similar patterns of restriction enzyme polymorphism .
	manualset3
104689	1	401571	13	NULL	NULL	0	NULL	41-Fold increase 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	41-Fold increase in creatine kinase has been reported .
	manualset3
104690	2	401571	13	NULL	NULL	0	NULL	creatine kinase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	41-Fold increase in creatine kinase has been reported .
	manualset3
104691	1	401572	13	NULL	NULL	0	NULL	Invitro studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Invitro studies on ectodomain shedding of type XVII collagen have also provided basic knowledge on the development of bullous pemphigoid .
	manualset3
104692	2	401572	13	NULL	NULL	0	NULL	ectodomain shedding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Invitro studies on ectodomain shedding of type XVII collagen have also provided basic knowledge on the development of bullous pemphigoid .
	manualset3
104693	3	401572	13	NULL	NULL	0	NULL	type XVII collagen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Invitro studies on ectodomain shedding of type XVII collagen have also provided basic knowledge on the development of bullous pemphigoid .
	manualset3
104694	4	401572	13	NULL	NULL	0	NULL	basic knowledge	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Invitro studies on ectodomain shedding of type XVII collagen have also provided basic knowledge on the development of bullous pemphigoid .
	manualset3
104695	5	401572	13	NULL	NULL	0	NULL	development 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Invitro studies on ectodomain shedding of type XVII collagen have also provided basic knowledge on the development of bullous pemphigoid .
	manualset3
104696	6	401572	13	NULL	NULL	0	NULL	bullous pemphigoid	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Invitro studies on ectodomain shedding of type XVII collagen have also provided basic knowledge on the development of bullous pemphigoid .
	manualset3
104697	1	401573	13	NULL	NULL	0	NULL	Involvement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of Escherichia coli K-12 DNA polymerase I in the growth of bacteriophage Mu .
	manualset3
104698	2	401573	13	NULL	NULL	0	NULL	Escherichia coli K-12 DNA polymerase I 	protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of Escherichia coli K-12 DNA polymerase I in the growth of bacteriophage Mu .
	manualset3
104699	3	401573	13	NULL	NULL	0	NULL	 growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of Escherichia coli K-12 DNA polymerase I in the growth of bacteriophage Mu .
	manualset3
104700	4	401573	13	NULL	NULL	0	NULL	bacteriophage Mu	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of Escherichia coli K-12 DNA polymerase I in the growth of bacteriophage Mu .
	manualset3
104701	1	401574	13	NULL	NULL	0	NULL	Involvement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of Src tyrosine kinase and mitogen-activated protein kinase in the facilitation of calcium channels in rat nucleus of the tractus solitarius by angiotensin II .
	manualset3
104702	2	401574	13	NULL	NULL	0	NULL	Src tyrosine kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of Src tyrosine kinase and mitogen-activated protein kinase in the facilitation of calcium channels in rat nucleus of the tractus solitarius by angiotensin II .
	manualset3
104703	3	401574	13	NULL	NULL	0	NULL	mitogen-activated protein kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of Src tyrosine kinase and mitogen-activated protein kinase in the facilitation of calcium channels in rat nucleus of the tractus solitarius by angiotensin II .
	manualset3
104704	4	401574	13	NULL	NULL	0	NULL	facilitation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of Src tyrosine kinase and mitogen-activated protein kinase in the facilitation of calcium channels in rat nucleus of the tractus solitarius by angiotensin II .
	manualset3
104705	5	401574	13	NULL	NULL	0	NULL	calcium channels	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of Src tyrosine kinase and mitogen-activated protein kinase in the facilitation of calcium channels in rat nucleus of the tractus solitarius by angiotensin II .
	manualset3
104706	6	401574	13	NULL	NULL	0	NULL	rat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of Src tyrosine kinase and mitogen-activated protein kinase in the facilitation of calcium channels in rat nucleus of the tractus solitarius by angiotensin II .
	manualset3
104707	7	401574	13	NULL	NULL	0	NULL	nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of Src tyrosine kinase and mitogen-activated protein kinase in the facilitation of calcium channels in rat nucleus of the tractus solitarius by angiotensin II .
	manualset3
104708	8	401574	13	NULL	NULL	0	NULL	 tractus solitarius 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of Src tyrosine kinase and mitogen-activated protein kinase in the facilitation of calcium channels in rat nucleus of the tractus solitarius by angiotensin II .
	manualset3
104709	9	401574	13	NULL	NULL	0	NULL	angiotensin II 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of Src tyrosine kinase and mitogen-activated protein kinase in the facilitation of calcium channels in rat nucleus of the tractus solitarius by angiotensin II .
	manualset3
104710	1	401575	13	NULL	NULL	0	NULL	Involvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of double-stranded RNA-activated protein kinase in the synergistic activation of nuclear factor-kappaB by tumor necrosis factor-alpha and gamma-interferon in preneuronal cells .
	manualset3
104711	2	401575	13	NULL	NULL	0	NULL	double-stranded RNA-activated protein kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of double-stranded RNA-activated protein kinase in the synergistic activation of nuclear factor-kappaB by tumor necrosis factor-alpha and gamma-interferon in preneuronal cells .
	manualset3
104712	3	401575	13	NULL	NULL	0	NULL	synergistic activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of double-stranded RNA-activated protein kinase in the synergistic activation of nuclear factor-kappaB by tumor necrosis factor-alpha and gamma-interferon in preneuronal cells .
	manualset3
104713	4	401575	13	NULL	NULL	0	NULL	nuclear factor-kappaB	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of double-stranded RNA-activated protein kinase in the synergistic activation of nuclear factor-kappaB by tumor necrosis factor-alpha and gamma-interferon in preneuronal cells .
	manualset3
104714	5	401575	13	NULL	NULL	0	NULL	tumor necrosis factor-alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of double-stranded RNA-activated protein kinase in the synergistic activation of nuclear factor-kappaB by tumor necrosis factor-alpha and gamma-interferon in preneuronal cells .
	manualset3
104715	6	401575	13	NULL	NULL	0	NULL	gamma-interferon	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of double-stranded RNA-activated protein kinase in the synergistic activation of nuclear factor-kappaB by tumor necrosis factor-alpha and gamma-interferon in preneuronal cells .
	manualset3
104716	7	401575	13	NULL	NULL	0	NULL	preneuronal cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of double-stranded RNA-activated protein kinase in the synergistic activation of nuclear factor-kappaB by tumor necrosis factor-alpha and gamma-interferon in preneuronal cells .
	manualset3
104717	1	401576	13	NULL	NULL	0	NULL	Involvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of lipid transfer protein in onion allergy .
	manualset3
104718	2	401576	13	NULL	NULL	0	NULL	lipid transfer protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of lipid transfer protein in onion allergy .
	manualset3
104719	3	401576	13	NULL	NULL	0	NULL	onion allergy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of lipid transfer protein in onion allergy .
	manualset3
104720	1	401577	13	NULL	NULL	0	NULL	Involvement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of sperm head cytoskeleton in the process of capping was evident from potentiation of cap formation by cytoskeleton disrupting agents like cytochalasin B and D. Patching of antigen antibody complexes was not affected by either of the agents .
	manualset3
104721	2	401577	13	NULL	NULL	0	NULL	 sperm head cytoskeleton 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of sperm head cytoskeleton in the process of capping was evident from potentiation of cap formation by cytoskeleton disrupting agents like cytochalasin B and D. Patching of antigen antibody complexes was not affected by either of the agents .
	manualset3
104722	3	401577	13	NULL	NULL	NULL	NULL	process of capping 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Involvement of sperm head cytoskeleton in the process of capping was evident from potentiation of cap formation by cytoskeleton disrupting agents like cytochalasin B and D. Patching of antigen antibody complexes was not affected by either of the agents .
	manualset3
104723	4	401577	13	NULL	NULL	0	NULL	 potentiation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of sperm head cytoskeleton in the process of capping was evident from potentiation of cap formation by cytoskeleton disrupting agents like cytochalasin B and D. Patching of antigen antibody complexes was not affected by either of the agents .
	manualset3
104724	5	401577	13	NULL	NULL	0	NULL	cap formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of sperm head cytoskeleton in the process of capping was evident from potentiation of cap formation by cytoskeleton disrupting agents like cytochalasin B and D. Patching of antigen antibody complexes was not affected by either of the agents .
	manualset3
104725	6	401577	13	NULL	NULL	NULL	NULL	cytoskeleton disrupting agents	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Involvement of sperm head cytoskeleton in the process of capping was evident from potentiation of cap formation by cytoskeleton disrupting agents like cytochalasin B and D. Patching of antigen antibody complexes was not affected by either of the agents .
	manualset3
104726	7	401577	13	NULL	NULL	0	NULL	cytochalasin B	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of sperm head cytoskeleton in the process of capping was evident from potentiation of cap formation by cytoskeleton disrupting agents like cytochalasin B and D. Patching of antigen antibody complexes was not affected by either of the agents .
	manualset3
104727	8	401577	13	NULL	NULL	0	NULL	cytochalasin D	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of sperm head cytoskeleton in the process of capping was evident from potentiation of cap formation by cytoskeleton disrupting agents like cytochalasin B and D. Patching of antigen antibody complexes was not affected by either of the agents .
	manualset3
104728	9	401577	13	NULL	NULL	0	NULL	Patching	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of sperm head cytoskeleton in the process of capping was evident from potentiation of cap formation by cytoskeleton disrupting agents like cytochalasin B and D. Patching of antigen antibody complexes was not affected by either of the agents .
	manualset3
104729	10	401577	13	NULL	NULL	0	NULL	antigen antibody complexes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of sperm head cytoskeleton in the process of capping was evident from potentiation of cap formation by cytoskeleton disrupting agents like cytochalasin B and D. Patching of antigen antibody complexes was not affected by either of the agents .
	manualset3
104730	11	401577	13	NULL	NULL	0	NULL	agents 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of sperm head cytoskeleton in the process of capping was evident from potentiation of cap formation by cytoskeleton disrupting agents like cytochalasin B and D. Patching of antigen antibody complexes was not affected by either of the agents .
	manualset3
104731	1	401578	13	NULL	NULL	0	NULL	Involvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of the PI3K/AKT pathway in the hypoglycemic effects of saponins from Helicteres isora .
	manualset3
104732	2	401578	13	NULL	NULL	0	NULL	PI3K/AKT pathway 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of the PI3K/AKT pathway in the hypoglycemic effects of saponins from Helicteres isora .
	manualset3
104733	3	401578	13	NULL	NULL	0	NULL	hypoglycemic effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of the PI3K/AKT pathway in the hypoglycemic effects of saponins from Helicteres isora .
	manualset3
104734	4	401578	13	NULL	NULL	0	NULL	saponins 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of the PI3K/AKT pathway in the hypoglycemic effects of saponins from Helicteres isora .
	manualset3
104735	5	401578	13	NULL	NULL	0	NULL	Helicteres isora	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of the PI3K/AKT pathway in the hypoglycemic effects of saponins from Helicteres isora .
	manualset3
104736	1	401579	13	NULL	NULL	0	NULL	Involvement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of transcription factor p53 and leptin in control of porcine ovarian granulosa cell functions .
	manualset3
104737	2	401579	13	NULL	NULL	0	NULL	transcription factor p53	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of transcription factor p53 and leptin in control of porcine ovarian granulosa cell functions .
	manualset3
104738	3	401579	13	NULL	NULL	0	NULL	leptin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of transcription factor p53 and leptin in control of porcine ovarian granulosa cell functions .
	manualset3
104739	4	401579	13	NULL	NULL	0	NULL	control 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of transcription factor p53 and leptin in control of porcine ovarian granulosa cell functions .
	manualset3
104740	5	401579	13	NULL	NULL	0	NULL	porcine ovarian granulosa cell functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of transcription factor p53 and leptin in control of porcine ovarian granulosa cell functions .
	manualset3
104741	1	401580	13	NULL	NULL	0	NULL	Iodine-I25 episcleral plaque therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Iodine-I25 episcleral plaque therapy in uveal melanoma .
	manualset3
104742	2	401580	13	NULL	NULL	0	NULL	uveal melanoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Iodine-I25 episcleral plaque therapy in uveal melanoma .
	manualset3
104743	1	401581	13	NULL	NULL	0	NULL	Iodine-induced neonatal hypothyroidism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Iodine-induced neonatal hypothyroidism secondary to maternal seaweed consumption : a common practice in some Asian cultures to promote breast milk supply .
	manualset3
104744	2	401581	13	NULL	NULL	NULL	NULL	maternal seaweed consumption	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Iodine-induced neonatal hypothyroidism secondary to maternal seaweed consumption : a common practice in some Asian cultures to promote breast milk supply .
	manualset3
104745	3	401581	13	NULL	NULL	0	NULL	common practice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Iodine-induced neonatal hypothyroidism secondary to maternal seaweed consumption : a common practice in some Asian cultures to promote breast milk supply .
	manualset3
104746	4	401581	13	NULL	NULL	0	NULL	Asian cultures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Iodine-induced neonatal hypothyroidism secondary to maternal seaweed consumption : a common practice in some Asian cultures to promote breast milk supply .
	manualset3
104747	5	401581	13	NULL	NULL	0	NULL	breast milk 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Iodine-induced neonatal hypothyroidism secondary to maternal seaweed consumption : a common practice in some Asian cultures to promote breast milk supply .
	manualset3
104748	6	401581	13	NULL	NULL	0	NULL	supply 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Iodine-induced neonatal hypothyroidism secondary to maternal seaweed consumption : a common practice in some Asian cultures to promote breast milk supply .
	manualset3
104749	1	401582	13	NULL	NULL	NULL	NULL	Iodine 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Iodine egg yolk was fractionated into the following 3 fractions by Folch 's method : Protein ( IEY - P ) , water-soluble ( IEY - A ) and lipid ( IEY - L ) fractions .
	manualset3
104750	3	401582	13	NULL	NULL	NULL	NULL	3 fractions	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Iodine egg yolk was fractionated into the following 3 fractions by Folch 's method : Protein ( IEY - P ) , water-soluble ( IEY - A ) and lipid ( IEY - L ) fractions .
	manualset3
104751	2	401582	13	NULL	NULL	0	NULL	 egg yolk	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Iodine egg yolk was fractionated into the following 3 fractions by Folch 's method : Protein ( IEY - P ) , water-soluble ( IEY - A ) and lipid ( IEY - L ) fractions .
	manualset3
104752	4	401582	13	NULL	NULL	0	NULL	Folch 's method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Iodine egg yolk was fractionated into the following 3 fractions by Folch 's method : Protein ( IEY - P ) , water-soluble ( IEY - A ) and lipid ( IEY - L ) fractions .
	manualset3
104753	5	401582	13	NULL	NULL	0	NULL	Protein ( IEY - P ) fraction	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Iodine egg yolk was fractionated into the following 3 fractions by Folch 's method : Protein ( IEY - P ) , water-soluble ( IEY - A ) and lipid ( IEY - L ) fractions .
	manualset3
104754	6	401582	13	NULL	NULL	0	NULL	water-soluble ( IEY - A ) fraction	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Iodine egg yolk was fractionated into the following 3 fractions by Folch 's method : Protein ( IEY - P ) , water-soluble ( IEY - A ) and lipid ( IEY - L ) fractions .
	manualset3
104755	7	401582	13	NULL	NULL	0	NULL	lipid ( IEY - L ) fraction	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Iodine egg yolk was fractionated into the following 3 fractions by Folch 's method : Protein ( IEY - P ) , water-soluble ( IEY - A ) and lipid ( IEY - L ) fractions .
	manualset3
104756	1	401583	13	NULL	NULL	0	NULL	Ion-pairing reversed-phase liquid chromatography ( RPLC ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ion-pairing reversed-phase liquid chromatography ( RPLC ) was used to separate two polysulfonates , rutin nona ( H - ) sulfonate sodium and rutin deca ( H - ) sulfonate sodium , which have very similar chemical structures .
	manualset3
104757	2	401583	13	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ion-pairing reversed-phase liquid chromatography ( RPLC ) was used to separate two polysulfonates , rutin nona ( H - ) sulfonate sodium and rutin deca ( H - ) sulfonate sodium , which have very similar chemical structures .
	manualset3
104758	3	401583	13	NULL	NULL	0	NULL	polysulfonates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ion-pairing reversed-phase liquid chromatography ( RPLC ) was used to separate two polysulfonates , rutin nona ( H - ) sulfonate sodium and rutin deca ( H - ) sulfonate sodium , which have very similar chemical structures .
	manualset3
104759	4	401583	13	NULL	NULL	0	NULL	rutin nona ( H - ) sulfonate sodium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ion-pairing reversed-phase liquid chromatography ( RPLC ) was used to separate two polysulfonates , rutin nona ( H - ) sulfonate sodium and rutin deca ( H - ) sulfonate sodium , which have very similar chemical structures .
	manualset3
104760	5	401583	13	NULL	NULL	0	NULL	rutin deca ( H - ) sulfonate sodium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ion-pairing reversed-phase liquid chromatography ( RPLC ) was used to separate two polysulfonates , rutin nona ( H - ) sulfonate sodium and rutin deca ( H - ) sulfonate sodium , which have very similar chemical structures .
	manualset3
104761	6	401583	13	NULL	NULL	0	NULL	chemical structures	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Ion-pairing reversed-phase liquid chromatography ( RPLC ) was used to separate two polysulfonates , rutin nona ( H - ) sulfonate sodium and rutin deca ( H - ) sulfonate sodium , which have very similar chemical structures .
	manualset3
104762	1	401584	13	NULL	NULL	0	NULL	Ion transport 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ion transport across isolated ileal mucosa invaded by salmonella .
	manualset3
104763	2	401584	13	NULL	NULL	0	NULL	 ileal mucosa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ion transport across isolated ileal mucosa invaded by salmonella .
	manualset3
104764	3	401584	13	NULL	NULL	0	NULL	 salmonella 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ion transport across isolated ileal mucosa invaded by salmonella .
	manualset3
104765	1	401585	13	NULL	NULL	0	NULL	Ionic C60 complexes	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Ionic and neutral C60 complexes with coordination assemblies of metal tetraphenylporphyrins , MIITPP2 .
	manualset3
104766	2	401585	13	NULL	NULL	0	NULL	neutral C60 complexes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ionic and neutral C60 complexes with coordination assemblies of metal tetraphenylporphyrins , MIITPP2 .
	manualset3
104767	3	401585	13	NULL	NULL	0	NULL	 coordination assemblies	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ionic and neutral C60 complexes with coordination assemblies of metal tetraphenylporphyrins , MIITPP2 .
	manualset3
104768	4	401585	13	NULL	NULL	0	NULL	metal tetraphenylporphyrins 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ionic and neutral C60 complexes with coordination assemblies of metal tetraphenylporphyrins , MIITPP2 .
	manualset3
104769	5	401585	13	NULL	NULL	0	NULL	MIITPP2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ionic and neutral C60 complexes with coordination assemblies of metal tetraphenylporphyrins , MIITPP2 .
	manualset3
104770	1	401586	13	NULL	NULL	0	NULL	Ionizing radiation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Ionizing radiation is the most established risk factor for meningioma formation .
	manualset3
104771	2	401586	13	NULL	NULL	0	NULL	 risk factor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ionizing radiation is the most established risk factor for meningioma formation .
	manualset3
104772	3	401586	13	NULL	NULL	0	NULL	meningioma formation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ionizing radiation is the most established risk factor for meningioma formation .
	manualset3
104773	1	401587	13	NULL	NULL	0	NULL	Iontophoretic injection 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Iontophoretic injection of horseradish peroxidase ( HRP ) into the medial part of the facial nucleus resulted in retrograde labeling in the lateral midbrain tegmentum contralaterally which corresponded to the paralemniscal zone ( PL ) .
	manualset3
104774	2	401587	13	NULL	NULL	0	NULL	horseradish peroxidase ( HRP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Iontophoretic injection of horseradish peroxidase ( HRP ) into the medial part of the facial nucleus resulted in retrograde labeling in the lateral midbrain tegmentum contralaterally which corresponded to the paralemniscal zone ( PL ) .
	manualset3
104775	3	401587	13	NULL	NULL	0	NULL	medial part	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Iontophoretic injection of horseradish peroxidase ( HRP ) into the medial part of the facial nucleus resulted in retrograde labeling in the lateral midbrain tegmentum contralaterally which corresponded to the paralemniscal zone ( PL ) .
	manualset3
104776	4	401587	13	NULL	NULL	0	NULL	facial nucleus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Iontophoretic injection of horseradish peroxidase ( HRP ) into the medial part of the facial nucleus resulted in retrograde labeling in the lateral midbrain tegmentum contralaterally which corresponded to the paralemniscal zone ( PL ) .
	manualset3
104777	5	401587	13	NULL	NULL	0	NULL	retrograde labeling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Iontophoretic injection of horseradish peroxidase ( HRP ) into the medial part of the facial nucleus resulted in retrograde labeling in the lateral midbrain tegmentum contralaterally which corresponded to the paralemniscal zone ( PL ) .
	manualset3
104778	6	401587	13	NULL	NULL	0	NULL	lateral midbrain tegmentum 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Iontophoretic injection of horseradish peroxidase ( HRP ) into the medial part of the facial nucleus resulted in retrograde labeling in the lateral midbrain tegmentum contralaterally which corresponded to the paralemniscal zone ( PL ) .
	manualset3
104779	7	401587	13	NULL	NULL	0	NULL	paralemniscal zone ( PL )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Iontophoretic injection of horseradish peroxidase ( HRP ) into the medial part of the facial nucleus resulted in retrograde labeling in the lateral midbrain tegmentum contralaterally which corresponded to the paralemniscal zone ( PL ) .
	manualset3
104780	1	401588	13	NULL	NULL	0	NULL	42S RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	42S RNA ran as a homogeneous fraction on polyacrylamide gels ; the `` derived '' 26S RNA as well as `` natural '' 26S RNA from infected cultures showed similar electrophoretic patterns of heterogeneity .
	manualset3
104781	2	401588	13	NULL	NULL	0	NULL	homogeneous fraction	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	42S RNA ran as a homogeneous fraction on polyacrylamide gels ; the `` derived '' 26S RNA as well as `` natural '' 26S RNA from infected cultures showed similar electrophoretic patterns of heterogeneity .
	manualset3
104782	3	401588	13	NULL	NULL	0	NULL	polyacrylamide gels 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	42S RNA ran as a homogeneous fraction on polyacrylamide gels ; the `` derived '' 26S RNA as well as `` natural '' 26S RNA from infected cultures showed similar electrophoretic patterns of heterogeneity .
	manualset3
104783	4	401588	13	NULL	NULL	NULL	NULL	`` derived '' 26S RNA	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	42S RNA ran as a homogeneous fraction on polyacrylamide gels ; the `` derived '' 26S RNA as well as `` natural '' 26S RNA from infected cultures showed similar electrophoretic patterns of heterogeneity .
	manualset3
104784	5	401588	13	NULL	NULL	0	NULL	`` natural '' 26S RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	42S RNA ran as a homogeneous fraction on polyacrylamide gels ; the `` derived '' 26S RNA as well as `` natural '' 26S RNA from infected cultures showed similar electrophoretic patterns of heterogeneity .
	manualset3
104785	6	401588	13	NULL	NULL	0	NULL	cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	42S RNA ran as a homogeneous fraction on polyacrylamide gels ; the `` derived '' 26S RNA as well as `` natural '' 26S RNA from infected cultures showed similar electrophoretic patterns of heterogeneity .
	manualset3
104786	7	401588	13	NULL	NULL	0	NULL	electrophoretic patterns	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	42S RNA ran as a homogeneous fraction on polyacrylamide gels ; the `` derived '' 26S RNA as well as `` natural '' 26S RNA from infected cultures showed similar electrophoretic patterns of heterogeneity .
	manualset3
104787	8	401588	13	NULL	NULL	0	NULL	heterogeneity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	42S RNA ran as a homogeneous fraction on polyacrylamide gels ; the `` derived '' 26S RNA as well as `` natural '' 26S RNA from infected cultures showed similar electrophoretic patterns of heterogeneity .
	manualset3
104788	1	401589	13	NULL	NULL	0	NULL	Ipr1 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Ipr1 gene mediates innate immunity to tuberculosis .
	manualset3
104789	2	401589	13	NULL	NULL	0	NULL	 innate immunity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ipr1 gene mediates innate immunity to tuberculosis .
	manualset3
104790	3	401589	13	NULL	NULL	0	NULL	tuberculosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Ipr1 gene mediates innate immunity to tuberculosis .
	manualset3
104791	1	401590	13	NULL	NULL	0	NULL	Ipragliflozin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Ipragliflozin showed good pharmacokinetic properties following oral dosing , and dose-dependently increased urinary glucose excretion , which lasted for over 12h in normal mice .
	manualset3
104792	2	401590	13	NULL	NULL	0	NULL	 pharmacokinetic properties 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ipragliflozin showed good pharmacokinetic properties following oral dosing , and dose-dependently increased urinary glucose excretion , which lasted for over 12h in normal mice .
	manualset3
104793	3	401590	13	NULL	NULL	0	NULL	oral dosing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ipragliflozin showed good pharmacokinetic properties following oral dosing , and dose-dependently increased urinary glucose excretion , which lasted for over 12h in normal mice .
	manualset3
104794	4	401590	13	NULL	NULL	0	NULL	urinary glucose excretion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ipragliflozin showed good pharmacokinetic properties following oral dosing , and dose-dependently increased urinary glucose excretion , which lasted for over 12h in normal mice .
	manualset3
104795	5	401590	13	NULL	NULL	0	NULL	12h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Ipragliflozin showed good pharmacokinetic properties following oral dosing , and dose-dependently increased urinary glucose excretion , which lasted for over 12h in normal mice .
	manualset3
104796	6	401590	13	NULL	NULL	0	NULL	normal mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ipragliflozin showed good pharmacokinetic properties following oral dosing , and dose-dependently increased urinary glucose excretion , which lasted for over 12h in normal mice .
	manualset3
104928	1	401591	13	NULL	NULL	NULL	NULL	Irinotecan/fluorouracil combination	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Irinotecan/fluorouracil combination in first-line therapy of older and younger patients with metastatic colorectal cancer : combined analysis of 2 , 691 patients in randomized controlled trials .
	manualset3
104931	4	401591	13	NULL	NULL	0	NULL	first-line therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Irinotecan/fluorouracil combination in first-line therapy of older and younger patients with metastatic colorectal cancer : combined analysis of 2 , 691 patients in randomized controlled trials .
	manualset3
104932	5	401591	13	NULL	NULL	0	NULL	older patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Irinotecan/fluorouracil combination in first-line therapy of older and younger patients with metastatic colorectal cancer : combined analysis of 2 , 691 patients in randomized controlled trials .
	manualset3
104933	6	401591	13	NULL	NULL	0	NULL	younger patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Irinotecan/fluorouracil combination in first-line therapy of older and younger patients with metastatic colorectal cancer : combined analysis of 2 , 691 patients in randomized controlled trials .
	manualset3
104934	7	401591	13	NULL	NULL	0	NULL	 metastatic colorectal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Irinotecan/fluorouracil combination in first-line therapy of older and younger patients with metastatic colorectal cancer : combined analysis of 2 , 691 patients in randomized controlled trials .
	manualset3
104935	8	401591	13	NULL	NULL	NULL	NULL	analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Irinotecan/fluorouracil combination in first-line therapy of older and younger patients with metastatic colorectal cancer : combined analysis of 2 , 691 patients in randomized controlled trials .
	manualset3
104936	9	401591	13	NULL	NULL	0	NULL	2 , 691	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Irinotecan/fluorouracil combination in first-line therapy of older and younger patients with metastatic colorectal cancer : combined analysis of 2 , 691 patients in randomized controlled trials .
	manualset3
104937	10	401591	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Irinotecan/fluorouracil combination in first-line therapy of older and younger patients with metastatic colorectal cancer : combined analysis of 2 , 691 patients in randomized controlled trials .
	manualset3
104938	11	401591	13	NULL	NULL	0	NULL	trials	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Irinotecan/fluorouracil combination in first-line therapy of older and younger patients with metastatic colorectal cancer : combined analysis of 2 , 691 patients in randomized controlled trials .
	manualset3
104939	1	401592	13	NULL	NULL	0	NULL	Iron-dependent amplification	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Iron-dependent amplification of the vascular effects of homocysteine may be one of several mechanisms by which stored iron increases cardiac risk .
	manualset3
104940	2	401592	13	NULL	NULL	0	NULL	vascular effects 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Iron-dependent amplification of the vascular effects of homocysteine may be one of several mechanisms by which stored iron increases cardiac risk .
	manualset3
104941	3	401592	13	NULL	NULL	0	NULL	homocysteine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Iron-dependent amplification of the vascular effects of homocysteine may be one of several mechanisms by which stored iron increases cardiac risk .
	manualset3
104942	4	401592	13	NULL	NULL	0	NULL	mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Iron-dependent amplification of the vascular effects of homocysteine may be one of several mechanisms by which stored iron increases cardiac risk .
	manualset3
104943	5	401592	13	NULL	NULL	0	NULL	 iron 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Iron-dependent amplification of the vascular effects of homocysteine may be one of several mechanisms by which stored iron increases cardiac risk .
	manualset3
104944	6	401592	13	NULL	NULL	0	NULL	increases cardiac risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Iron-dependent amplification of the vascular effects of homocysteine may be one of several mechanisms by which stored iron increases cardiac risk .
	manualset3
104945	1	401593	13	NULL	NULL	NULL	NULL	Iron	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Iron Loading and Overloading due to Ineffective Erythropoiesis .
	manualset3
104946	2	401593	13	NULL	NULL	0	NULL	Loading	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Iron Loading and Overloading due to Ineffective Erythropoiesis .
	manualset3
104947	3	401593	13	NULL	NULL	0	NULL	Overloading	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Iron Loading and Overloading due to Ineffective Erythropoiesis .
	manualset3
104948	4	401593	13	NULL	NULL	0	NULL	Ineffective Erythropoiesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Iron Loading and Overloading due to Ineffective Erythropoiesis .
	manualset3
104949	1	401594	13	NULL	NULL	0	NULL	Iron	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Iron administration to young rats significantly increased hepatic iron content and ferritin but did not affect markers of lipid peroxidation under control conditions or after heat stress .
	manualset3
104950	2	401594	13	NULL	NULL	0	NULL	 administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Iron administration to young rats significantly increased hepatic iron content and ferritin but did not affect markers of lipid peroxidation under control conditions or after heat stress .
	manualset3
104951	3	401594	13	NULL	NULL	0	NULL	young rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Iron administration to young rats significantly increased hepatic iron content and ferritin but did not affect markers of lipid peroxidation under control conditions or after heat stress .
	manualset3
104952	4	401594	13	NULL	NULL	0	NULL	hepatic iron content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Iron administration to young rats significantly increased hepatic iron content and ferritin but did not affect markers of lipid peroxidation under control conditions or after heat stress .
	manualset3
104953	5	401594	13	NULL	NULL	0	NULL	ferritin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Iron administration to young rats significantly increased hepatic iron content and ferritin but did not affect markers of lipid peroxidation under control conditions or after heat stress .
	manualset3
104954	6	401594	13	NULL	NULL	0	NULL	markers 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Iron administration to young rats significantly increased hepatic iron content and ferritin but did not affect markers of lipid peroxidation under control conditions or after heat stress .
	manualset3
104955	7	401594	13	NULL	NULL	0	NULL	lipid peroxidation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Iron administration to young rats significantly increased hepatic iron content and ferritin but did not affect markers of lipid peroxidation under control conditions or after heat stress .
	manualset3
104956	8	401594	13	NULL	NULL	0	NULL	control conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Iron administration to young rats significantly increased hepatic iron content and ferritin but did not affect markers of lipid peroxidation under control conditions or after heat stress .
	manualset3
104957	9	401594	13	NULL	NULL	0	NULL	heat stress	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Iron administration to young rats significantly increased hepatic iron content and ferritin but did not affect markers of lipid peroxidation under control conditions or after heat stress .
	manualset3
104958	1	401595	13	NULL	NULL	0	NULL	Iron overload	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Iron overload and heart fibrosis in mice deficient for both beta2-microglobulin and Rag1 .
	manualset3
104959	2	401595	13	NULL	NULL	0	NULL	heart fibrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Iron overload and heart fibrosis in mice deficient for both beta2-microglobulin and Rag1 .
	manualset3
104960	3	401595	13	NULL	NULL	0	NULL	 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Iron overload and heart fibrosis in mice deficient for both beta2-microglobulin and Rag1 .
	manualset3
104961	4	401595	13	NULL	NULL	0	NULL	beta2-microglobulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Iron overload and heart fibrosis in mice deficient for both beta2-microglobulin and Rag1 .
	manualset3
104962	5	401595	13	NULL	NULL	NULL	NULL	Rag1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Iron overload and heart fibrosis in mice deficient for both beta2-microglobulin and Rag1 .
	manualset3
104963	1	401596	13	NULL	NULL	0	NULL	 uveal melanomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Irradiated uveal melanomas : cytopathologic correlation with prognosis .
	manualset3
104964	2	401596	13	NULL	NULL	0	NULL	cytopathologic correlation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Irradiated uveal melanomas : cytopathologic correlation with prognosis .
	manualset3
104965	3	401596	13	NULL	NULL	0	NULL	prognosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Irradiated uveal melanomas : cytopathologic correlation with prognosis .
	manualset3
104966	1	401597	13	NULL	NULL	0	NULL	43 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	43 patients ( 81.1 % ) had P. falciparum and 10 patients ( 18.9 % ) had P. vivax .
	manualset3
104967	2	401597	13	NULL	NULL	0	NULL	81.1 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	43 patients ( 81.1 % ) had P. falciparum and 10 patients ( 18.9 % ) had P. vivax .
	manualset3
104968	3	401597	13	NULL	NULL	0	NULL	P. falciparum 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	43 patients ( 81.1 % ) had P. falciparum and 10 patients ( 18.9 % ) had P. vivax .
	manualset3
104969	4	401597	13	NULL	NULL	0	NULL	10 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	43 patients ( 81.1 % ) had P. falciparum and 10 patients ( 18.9 % ) had P. vivax .
	manualset3
104970	5	401597	13	NULL	NULL	0	NULL	 18.9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	43 patients ( 81.1 % ) had P. falciparum and 10 patients ( 18.9 % ) had P. vivax .
	manualset3
104971	6	401597	13	NULL	NULL	0	NULL	P. vivax	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	43 patients ( 81.1 % ) had P. falciparum and 10 patients ( 18.9 % ) had P. vivax .
	manualset3
104972	1	401598	13	NULL	NULL	NULL	NULL	Irradiation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Irradiation may result in a greater frequency of live ( albeit incapable of resulting in an infestation ) larvae being found than would be expected compared with other treatments that provide acute mortality .
	manualset3
104973	2	401598	13	NULL	NULL	0	NULL	frequency	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Irradiation may result in a greater frequency of live ( albeit incapable of resulting in an infestation ) larvae being found than would be expected compared with other treatments that provide acute mortality .
	manualset3
104974	3	401598	13	NULL	NULL	0	NULL	incapable	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Irradiation may result in a greater frequency of live ( albeit incapable of resulting in an infestation ) larvae being found than would be expected compared with other treatments that provide acute mortality .
	manualset3
104975	4	401598	13	NULL	NULL	0	NULL	infestation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Irradiation may result in a greater frequency of live ( albeit incapable of resulting in an infestation ) larvae being found than would be expected compared with other treatments that provide acute mortality .
	manualset3
104976	5	401598	13	NULL	NULL	0	NULL	larvae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Irradiation may result in a greater frequency of live ( albeit incapable of resulting in an infestation ) larvae being found than would be expected compared with other treatments that provide acute mortality .
	manualset3
104977	6	401598	13	NULL	NULL	NULL	NULL	 treatments	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Irradiation may result in a greater frequency of live ( albeit incapable of resulting in an infestation ) larvae being found than would be expected compared with other treatments that provide acute mortality .
	manualset3
104978	7	401598	13	NULL	NULL	0	NULL	acute mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Irradiation may result in a greater frequency of live ( albeit incapable of resulting in an infestation ) larvae being found than would be expected compared with other treatments that provide acute mortality .
	manualset3
104979	1	401599	13	NULL	NULL	0	NULL	Irradiation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Irradiation affected axonal growth , differentiation of Schwann cells and formation of a perineurium .
	manualset3
104980	2	401599	13	NULL	NULL	0	NULL	axonal growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Irradiation affected axonal growth , differentiation of Schwann cells and formation of a perineurium .
	manualset3
104981	3	401599	13	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Irradiation affected axonal growth , differentiation of Schwann cells and formation of a perineurium .
	manualset3
104982	4	401599	13	NULL	NULL	0	NULL	Schwann cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Irradiation affected axonal growth , differentiation of Schwann cells and formation of a perineurium .
	manualset3
104983	5	401599	13	NULL	NULL	0	NULL	formation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Irradiation affected axonal growth , differentiation of Schwann cells and formation of a perineurium .
	manualset3
104984	6	401599	13	NULL	NULL	0	NULL	perineurium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Irradiation affected axonal growth , differentiation of Schwann cells and formation of a perineurium .
	manualset3
104985	1	401600	13	NULL	NULL	0	NULL	Irregular bleeding 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Irregular bleeding in women : causes and nursing intervention .
	manualset3
104986	2	401600	13	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Irregular bleeding in women : causes and nursing intervention .
	manualset3
104987	3	401600	13	NULL	NULL	0	NULL	 causes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Irregular bleeding in women : causes and nursing intervention .
	manualset3
104988	4	401600	13	NULL	NULL	0	NULL	nursing intervention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Irregular bleeding in women : causes and nursing intervention .
	manualset3
104989	1	401601	13	NULL	NULL	0	NULL	CaMKII	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Is CaMKII a link between inflammation and hypertrophy in heart ?
	manualset3
104990	2	401601	13	NULL	NULL	0	NULL	link	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Is CaMKII a link between inflammation and hypertrophy in heart ?
	manualset3
104991	3	401601	13	NULL	NULL	0	NULL	inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Is CaMKII a link between inflammation and hypertrophy in heart ?
	manualset3
104992	4	401601	13	NULL	NULL	0	NULL	hypertrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Is CaMKII a link between inflammation and hypertrophy in heart ?
	manualset3
104993	5	401601	13	NULL	NULL	0	NULL	heart	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Is CaMKII a link between inflammation and hypertrophy in heart ?
	manualset3
104994	1	401602	13	NULL	NULL	0	NULL	detection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Is detection of melanoma metastasis during surveillance in an early phase of development associated with a survival benefit ?
	manualset3
104995	2	401602	13	NULL	NULL	0	NULL	melanoma metastasis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Is detection of melanoma metastasis during surveillance in an early phase of development associated with a survival benefit ?
	manualset3
104996	3	401602	13	NULL	NULL	0	NULL	surveillance	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Is detection of melanoma metastasis during surveillance in an early phase of development associated with a survival benefit ?
	manualset3
104997	4	401602	13	NULL	NULL	0	NULL	early phase 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Is detection of melanoma metastasis during surveillance in an early phase of development associated with a survival benefit ?
	manualset3
104998	5	401602	13	NULL	NULL	0	NULL	development	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Is detection of melanoma metastasis during surveillance in an early phase of development associated with a survival benefit ?
	manualset3
104999	6	401602	13	NULL	NULL	0	NULL	survival benefit	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Is detection of melanoma metastasis during surveillance in an early phase of development associated with a survival benefit ?
	manualset3
105000	1	401603	13	NULL	NULL	0	NULL	 functional capacity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Is functional capacity evaluation useful in preplacement examinations ?
	manualset3
105001	2	401603	13	NULL	NULL	0	NULL	evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Is functional capacity evaluation useful in preplacement examinations ?
	manualset3
105002	3	401603	13	NULL	NULL	0	NULL	preplacement examinations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Is functional capacity evaluation useful in preplacement examinations ?
	manualset3
105003	1	401604	13	NULL	NULL	0	NULL	 hypothalamic prostaglandin E2	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Is hypothalamic prostaglandin E2 involved in avian fever ?
	manualset3
105004	2	401604	13	NULL	NULL	0	NULL	avian fever	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Is hypothalamic prostaglandin E2 involved in avian fever ?
	manualset3
105005	1	401605	13	NULL	NULL	0	NULL	nitric oxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Is nitric oxide involved in the pathophysiology of essential hyperhidrosis ?
	manualset3
105006	2	401605	13	NULL	NULL	0	NULL	pathophysiology 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Is nitric oxide involved in the pathophysiology of essential hyperhidrosis ?
	manualset3
105007	3	401605	13	NULL	NULL	0	NULL	hyperhidrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Is nitric oxide involved in the pathophysiology of essential hyperhidrosis ?
	manualset3
105008	1	401606	13	NULL	NULL	0	NULL	osseous dysplasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Is osseous dysplasia a primary feature of neurofibromatosis 1 ( NF1 ) ?
	manualset3
105009	2	401606	13	NULL	NULL	0	NULL	primary feature	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Is osseous dysplasia a primary feature of neurofibromatosis 1 ( NF1 ) ?
	manualset3
105010	3	401606	13	NULL	NULL	0	NULL	neurofibromatosis 1 ( NF1 ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Is osseous dysplasia a primary feature of neurofibromatosis 1 ( NF1 ) ?
	manualset3
105011	1	401607	13	NULL	NULL	0	NULL	spa therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Is spa therapy cost-effective in rheumatic disorders ?
	manualset3
105012	2	401607	13	NULL	NULL	0	NULL	rheumatic disorders 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Is spa therapy cost-effective in rheumatic disorders ?
	manualset3
105013	1	401608	13	NULL	NULL	0	NULL	Internet	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Is the Internet a reliable source for dietary recommendations for stone formers ?
	manualset3
105014	2	401608	13	NULL	NULL	0	NULL	reliable source	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Is the Internet a reliable source for dietary recommendations for stone formers ?
	manualset3
105015	3	401608	13	NULL	NULL	0	NULL	dietary recommendations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Is the Internet a reliable source for dietary recommendations for stone formers ?
	manualset3
105016	4	401608	13	NULL	NULL	0	NULL	stone formers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Is the Internet a reliable source for dietary recommendations for stone formers ?
	manualset3
105017	1	401609	13	NULL	NULL	0	NULL	medial wall 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Is the medial wall of the intercondylar notch useful for tibial rotational reference in unicompartmental knee arthroplasty ?
	manualset3
105018	2	401609	13	NULL	NULL	0	NULL	intercondylar notch	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Is the medial wall of the intercondylar notch useful for tibial rotational reference in unicompartmental knee arthroplasty ?
	manualset3
105019	3	401609	13	NULL	NULL	NULL	NULL	reference 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Is the medial wall of the intercondylar notch useful for tibial rotational reference in unicompartmental knee arthroplasty ?
	manualset3
105020	4	401609	13	NULL	NULL	0	NULL	knee arthroplasty 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Is the medial wall of the intercondylar notch useful for tibial rotational reference in unicompartmental knee arthroplasty ?
	manualset3
105021	1	401610	13	NULL	NULL	0	NULL	site of action	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Is the site of action of grayanotoxin the sodium channel gating of squid axon ?
	manualset3
105022	2	401610	13	NULL	NULL	0	NULL	grayanotoxin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Is the site of action of grayanotoxin the sodium channel gating of squid axon ?
	manualset3
105023	3	401610	13	NULL	NULL	0	NULL	sodium channel gating	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Is the site of action of grayanotoxin the sodium channel gating of squid axon ?
	manualset3
105024	4	401610	13	NULL	NULL	0	NULL	squid axon	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Is the site of action of grayanotoxin the sodium channel gating of squid axon ?
	manualset3
105025	1	401611	13	NULL	NULL	0	NULL	 use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Is the use of sunscreens a risk factor for malignant melanoma ?
	manualset3
105026	2	401611	13	NULL	NULL	0	NULL	sunscreens 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Is the use of sunscreens a risk factor for malignant melanoma ?
	manualset3
105027	3	401611	13	NULL	NULL	0	NULL	risk factor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Is the use of sunscreens a risk factor for malignant melanoma ?
	manualset3
105028	4	401611	13	NULL	NULL	0	NULL	malignant melanoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Is the use of sunscreens a risk factor for malignant melanoma ?
	manualset3
105029	1	401612	13	NULL	NULL	NULL	NULL	445 women 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	445 women ( 188 HIV + 257 HIV - ) residing in an urban low income area were interviewed regarding current IPV experiences ( no IPV , IPV more than 1 year ago , IPV in last year ) , HIV status ( positive and negative ) , use of illicit drugs , and presence of instrumental social support .
	manualset3
105030	2	401612	13	NULL	NULL	NULL	NULL	188 HIV +	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	445 women ( 188 HIV + 257 HIV - ) residing in an urban low income area were interviewed regarding current IPV experiences ( no IPV , IPV more than 1 year ago , IPV in last year ) , HIV status ( positive and negative ) , use of illicit drugs , and presence of instrumental social support .
	manualset3
105031	3	401612	13	NULL	NULL	0	NULL	257 HIV -	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	445 women ( 188 HIV + 257 HIV - ) residing in an urban low income area were interviewed regarding current IPV experiences ( no IPV , IPV more than 1 year ago , IPV in last year ) , HIV status ( positive and negative ) , use of illicit drugs , and presence of instrumental social support .
	manualset3
105032	4	401612	13	NULL	NULL	0	NULL	urban low income area 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	445 women ( 188 HIV + 257 HIV - ) residing in an urban low income area were interviewed regarding current IPV experiences ( no IPV , IPV more than 1 year ago , IPV in last year ) , HIV status ( positive and negative ) , use of illicit drugs , and presence of instrumental social support .
	manualset3
105033	5	401612	13	NULL	NULL	0	NULL	IPV experiences	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	445 women ( 188 HIV + 257 HIV - ) residing in an urban low income area were interviewed regarding current IPV experiences ( no IPV , IPV more than 1 year ago , IPV in last year ) , HIV status ( positive and negative ) , use of illicit drugs , and presence of instrumental social support .
	manualset3
105034	6	401612	13	NULL	NULL	0	NULL	no IPV 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	445 women ( 188 HIV + 257 HIV - ) residing in an urban low income area were interviewed regarding current IPV experiences ( no IPV , IPV more than 1 year ago , IPV in last year ) , HIV status ( positive and negative ) , use of illicit drugs , and presence of instrumental social support .
	manualset3
105035	7	401612	13	NULL	NULL	0	NULL	 IPV	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	445 women ( 188 HIV + 257 HIV - ) residing in an urban low income area were interviewed regarding current IPV experiences ( no IPV , IPV more than 1 year ago , IPV in last year ) , HIV status ( positive and negative ) , use of illicit drugs , and presence of instrumental social support .
	manualset3
105036	8	401612	13	NULL	NULL	0	NULL	more than 1 year ago 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	445 women ( 188 HIV + 257 HIV - ) residing in an urban low income area were interviewed regarding current IPV experiences ( no IPV , IPV more than 1 year ago , IPV in last year ) , HIV status ( positive and negative ) , use of illicit drugs , and presence of instrumental social support .
	manualset3
105037	9	401612	13	NULL	NULL	0	NULL	IPV	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	445 women ( 188 HIV + 257 HIV - ) residing in an urban low income area were interviewed regarding current IPV experiences ( no IPV , IPV more than 1 year ago , IPV in last year ) , HIV status ( positive and negative ) , use of illicit drugs , and presence of instrumental social support .
	manualset3
105038	10	401612	13	NULL	NULL	0	NULL	last year 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	445 women ( 188 HIV + 257 HIV - ) residing in an urban low income area were interviewed regarding current IPV experiences ( no IPV , IPV more than 1 year ago , IPV in last year ) , HIV status ( positive and negative ) , use of illicit drugs , and presence of instrumental social support .
	manualset3
105039	11	401612	13	NULL	NULL	0	NULL	HIV status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	445 women ( 188 HIV + 257 HIV - ) residing in an urban low income area were interviewed regarding current IPV experiences ( no IPV , IPV more than 1 year ago , IPV in last year ) , HIV status ( positive and negative ) , use of illicit drugs , and presence of instrumental social support .
	manualset3
105040	12	401612	13	NULL	NULL	0	NULL	positive	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	445 women ( 188 HIV + 257 HIV - ) residing in an urban low income area were interviewed regarding current IPV experiences ( no IPV , IPV more than 1 year ago , IPV in last year ) , HIV status ( positive and negative ) , use of illicit drugs , and presence of instrumental social support .
	manualset3
105041	13	401612	13	NULL	NULL	0	NULL	negative	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	445 women ( 188 HIV + 257 HIV - ) residing in an urban low income area were interviewed regarding current IPV experiences ( no IPV , IPV more than 1 year ago , IPV in last year ) , HIV status ( positive and negative ) , use of illicit drugs , and presence of instrumental social support .
	manualset3
105042	14	401612	13	NULL	NULL	0	NULL	 use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	445 women ( 188 HIV + 257 HIV - ) residing in an urban low income area were interviewed regarding current IPV experiences ( no IPV , IPV more than 1 year ago , IPV in last year ) , HIV status ( positive and negative ) , use of illicit drugs , and presence of instrumental social support .
	manualset3
105043	15	401612	13	NULL	NULL	0	NULL	illicit drugs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	445 women ( 188 HIV + 257 HIV - ) residing in an urban low income area were interviewed regarding current IPV experiences ( no IPV , IPV more than 1 year ago , IPV in last year ) , HIV status ( positive and negative ) , use of illicit drugs , and presence of instrumental social support .
	manualset3
105044	16	401612	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	445 women ( 188 HIV + 257 HIV - ) residing in an urban low income area were interviewed regarding current IPV experiences ( no IPV , IPV more than 1 year ago , IPV in last year ) , HIV status ( positive and negative ) , use of illicit drugs , and presence of instrumental social support .
	manualset3
105045	17	401612	13	NULL	NULL	0	NULL	social support	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	445 women ( 188 HIV + 257 HIV - ) residing in an urban low income area were interviewed regarding current IPV experiences ( no IPV , IPV more than 1 year ago , IPV in last year ) , HIV status ( positive and negative ) , use of illicit drugs , and presence of instrumental social support .
	manualset3
105046	1	401613	13	NULL	NULL	0	NULL	niche	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Is there a niche for DNA microarrays in molecular diagnostics ?
	manualset3
105047	2	401613	13	NULL	NULL	0	NULL	DNA microarrays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Is there a niche for DNA microarrays in molecular diagnostics ?
	manualset3
105048	3	401613	13	NULL	NULL	0	NULL	molecular diagnostics 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Is there a niche for DNA microarrays in molecular diagnostics ?
	manualset3
105049	1	401614	13	NULL	NULL	0	NULL	role 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Is there a role for antibiotics in the treatment of patients with rheumatoid arthritis ?
	manualset3
105050	2	401614	13	NULL	NULL	0	NULL	antibiotics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Is there a role for antibiotics in the treatment of patients with rheumatoid arthritis ?
	manualset3
105051	3	401614	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Is there a role for antibiotics in the treatment of patients with rheumatoid arthritis ?
	manualset3
105052	4	401614	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Is there a role for antibiotics in the treatment of patients with rheumatoid arthritis ?
	manualset3
105053	5	401614	13	NULL	NULL	0	NULL	rheumatoid arthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Is there a role for antibiotics in the treatment of patients with rheumatoid arthritis ?
	manualset3
105054	1	401615	13	NULL	NULL	0	NULL	practice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Is there an evidence-based practice for burns ?
	manualset3
105055	2	401615	13	NULL	NULL	0	NULL	burns	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Is there an evidence-based practice for burns ?
	manualset3
105056	1	401616	13	NULL	NULL	0	NULL	personal doctor	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Is there a personal doctor in the house ?
	manualset3
105057	2	401616	13	NULL	NULL	0	NULL	house	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Is there a personal doctor in the house ?
	manualset3
105058	1	401617	13	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Is there evidence that rotavirus vaccines are effective in preventing acute gastroenteritis complications such as dehydration and hospitalization ?
	manualset3
105059	2	401617	13	NULL	NULL	0	NULL	rotavirus vaccines	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Is there evidence that rotavirus vaccines are effective in preventing acute gastroenteritis complications such as dehydration and hospitalization ?
	manualset3
105060	3	401617	13	NULL	NULL	0	NULL	acute gastroenteritis complications 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Is there evidence that rotavirus vaccines are effective in preventing acute gastroenteritis complications such as dehydration and hospitalization ?
	manualset3
105061	4	401617	13	NULL	NULL	0	NULL	dehydration 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Is there evidence that rotavirus vaccines are effective in preventing acute gastroenteritis complications such as dehydration and hospitalization ?
	manualset3
105062	5	401617	13	NULL	NULL	0	NULL	hospitalization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Is there evidence that rotavirus vaccines are effective in preventing acute gastroenteritis complications such as dehydration and hospitalization ?
	manualset3
105063	1	401618	13	NULL	NULL	0	NULL	Ischemia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ischemia modified albumin has been reported to increase following percutaneous coronary intervention and in acute coronary syndromes .
	manualset3
105064	2	401618	13	NULL	NULL	0	NULL	albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Ischemia modified albumin has been reported to increase following percutaneous coronary intervention and in acute coronary syndromes .
	manualset3
105065	3	401618	13	NULL	NULL	0	NULL	percutaneous coronary intervention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ischemia modified albumin has been reported to increase following percutaneous coronary intervention and in acute coronary syndromes .
	manualset3
105066	4	401618	13	NULL	NULL	0	NULL	acute coronary syndromes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ischemia modified albumin has been reported to increase following percutaneous coronary intervention and in acute coronary syndromes .
	manualset3
105067	1	401619	13	NULL	NULL	0	NULL	Ischemic complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ischemic complications have been reduced to the point that bleeding has become the most common complication .
	manualset3
105068	2	401619	13	NULL	NULL	0	NULL	bleeding 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ischemic complications have been reduced to the point that bleeding has become the most common complication .
	manualset3
105069	3	401619	13	NULL	NULL	0	NULL	common complication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ischemic complications have been reduced to the point that bleeding has become the most common complication .
	manualset3
105070	1	401620	13	NULL	NULL	0	NULL	allograft ureter	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ischemic necrosis of the allograft ureter .
	manualset3
105071	2	401620	13	NULL	NULL	0	NULL	Ischemic necrosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ischemic necrosis of the allograft ureter .
	manualset3
105072	1	401621	13	NULL	NULL	0	NULL	Isoflavone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Isoflavone content of soya-based laboratory animal diets .
	manualset3
105073	2	401621	13	NULL	NULL	0	NULL	content 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isoflavone content of soya-based laboratory animal diets .
	manualset3
105074	3	401621	13	NULL	NULL	0	NULL	soya-based laboratory animal diets	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Isoflavone content of soya-based laboratory animal diets .
	manualset3
105075	1	401622	13	NULL	NULL	0	NULL	47-61-fold	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	47-61-fold selective for housefly vs rat GABA receptors .
	manualset3
105076	2	401622	13	NULL	NULL	NULL	NULL	housefly GABA receptors	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	47-61-fold selective for housefly vs rat GABA receptors .
	manualset3
105077	3	401622	13	NULL	NULL	NULL	NULL	rat GABA receptors	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	47-61-fold selective for housefly vs rat GABA receptors .
	manualset3
105078	1	401623	13	NULL	NULL	0	NULL	Isoflurane 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Isoflurane produced respiratory depression ; end tidal carbon dioxide tension increased from 38.8 + / - 3.6 mmHg at 1 % , to 42.6 + / - 4.3 mmHg and 48.8 + / - 4.9 mmHg at 1.5 and 2 % respectively .
	manualset3
105079	2	401623	13	NULL	NULL	0	NULL	respiratory depression 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Isoflurane produced respiratory depression ; end tidal carbon dioxide tension increased from 38.8 + / - 3.6 mmHg at 1 % , to 42.6 + / - 4.3 mmHg and 48.8 + / - 4.9 mmHg at 1.5 and 2 % respectively .
	manualset3
105080	3	401623	13	NULL	NULL	0	NULL	end tidal carbon dioxide tension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Isoflurane produced respiratory depression ; end tidal carbon dioxide tension increased from 38.8 + / - 3.6 mmHg at 1 % , to 42.6 + / - 4.3 mmHg and 48.8 + / - 4.9 mmHg at 1.5 and 2 % respectively .
	manualset3
105081	4	401623	13	NULL	NULL	0	NULL	38.8 + / - 3.6 mmHg at 1 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Isoflurane produced respiratory depression ; end tidal carbon dioxide tension increased from 38.8 + / - 3.6 mmHg at 1 % , to 42.6 + / - 4.3 mmHg and 48.8 + / - 4.9 mmHg at 1.5 and 2 % respectively .
	manualset3
105082	5	401623	13	NULL	NULL	0	NULL	 42.6 + / - 4.3 mmHg at 1.5 %  	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Isoflurane produced respiratory depression ; end tidal carbon dioxide tension increased from 38.8 + / - 3.6 mmHg at 1 % , to 42.6 + / - 4.3 mmHg and 48.8 + / - 4.9 mmHg at 1.5 and 2 % respectively .
	manualset3
105083	6	401623	13	NULL	NULL	0	NULL	48.8 + / - 4.9 mmHg at 2 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Isoflurane produced respiratory depression ; end tidal carbon dioxide tension increased from 38.8 + / - 3.6 mmHg at 1 % , to 42.6 + / - 4.3 mmHg and 48.8 + / - 4.9 mmHg at 1.5 and 2 % respectively .
	manualset3
105084	1	401624	13	NULL	NULL	0	NULL	H9/HTLV-IIIRf	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolate H9/HTLV-IIIRf was nonstimulatory on a B cell preparation containing LDC and suppressive on LDC accessory function yet could enhance function of B cells when the LDC were depleted .
	manualset3
105085	2	401624	13	NULL	NULL	0	NULL	B cell preparation	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolate H9/HTLV-IIIRf was nonstimulatory on a B cell preparation containing LDC and suppressive on LDC accessory function yet could enhance function of B cells when the LDC were depleted .
	manualset3
105086	3	401624	13	NULL	NULL	0	NULL	LDC 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolate H9/HTLV-IIIRf was nonstimulatory on a B cell preparation containing LDC and suppressive on LDC accessory function yet could enhance function of B cells when the LDC were depleted .
	manualset3
105087	4	401624	13	NULL	NULL	0	NULL	LDC accessory function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolate H9/HTLV-IIIRf was nonstimulatory on a B cell preparation containing LDC and suppressive on LDC accessory function yet could enhance function of B cells when the LDC were depleted .
	manualset3
105088	5	401624	13	NULL	NULL	0	NULL	function of B cells	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolate H9/HTLV-IIIRf was nonstimulatory on a B cell preparation containing LDC and suppressive on LDC accessory function yet could enhance function of B cells when the LDC were depleted .
	manualset3
105089	6	401624	13	NULL	NULL	0	NULL	LDC 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolate H9/HTLV-IIIRf was nonstimulatory on a B cell preparation containing LDC and suppressive on LDC accessory function yet could enhance function of B cells when the LDC were depleted .
	manualset3
105090	1	401625	13	NULL	NULL	0	NULL	keratinocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolated keratinocytes display several distinct stages leading to terminal maturation .
	manualset3
105091	2	401625	13	NULL	NULL	0	NULL	distinct stages 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolated keratinocytes display several distinct stages leading to terminal maturation .
	manualset3
105092	3	401625	13	NULL	NULL	0	NULL	terminal maturation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolated keratinocytes display several distinct stages leading to terminal maturation .
	manualset3
105093	1	401626	13	NULL	NULL	NULL	NULL	rat liver mitochondria	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Isolated rat liver mitochondria were incubated with vitamin C , resveratrol and lipoic acid .
	manualset3
105094	2	401626	13	NULL	NULL	0	NULL	vitamin C	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolated rat liver mitochondria were incubated with vitamin C , resveratrol and lipoic acid .
	manualset3
105095	3	401626	13	NULL	NULL	0	NULL	resveratrol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolated rat liver mitochondria were incubated with vitamin C , resveratrol and lipoic acid .
	manualset3
105096	4	401626	13	NULL	NULL	NULL	NULL	lipoic acid	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Isolated rat liver mitochondria were incubated with vitamin C , resveratrol and lipoic acid .
	manualset3
105097	1	401627	13	NULL	NULL	0	NULL	single-molecule magnets 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolated single-molecule magnets on native gold .
	manualset3
105098	2	401627	13	NULL	NULL	0	NULL	native gold	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolated single-molecule magnets on native gold .
	manualset3
105099	1	401628	13	NULL	NULL	0	NULL	Isolates 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolates expressing MR/K hemagglutinin bound in higher numbers to catheter material ( P = .023 ) than did those not expressing this hemagglutinin .
	manualset3
105100	2	401628	13	NULL	NULL	0	NULL	MR/K hemagglutinin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolates expressing MR/K hemagglutinin bound in higher numbers to catheter material ( P = .023 ) than did those not expressing this hemagglutinin .
	manualset3
105101	3	401628	13	NULL	NULL	0	NULL	numbers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolates expressing MR/K hemagglutinin bound in higher numbers to catheter material ( P = .023 ) than did those not expressing this hemagglutinin .
	manualset3
105102	4	401628	13	NULL	NULL	0	NULL	catheter material	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolates expressing MR/K hemagglutinin bound in higher numbers to catheter material ( P = .023 ) than did those not expressing this hemagglutinin .
	manualset3
105103	5	401628	13	NULL	NULL	0	NULL	P = .023	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolates expressing MR/K hemagglutinin bound in higher numbers to catheter material ( P = .023 ) than did those not expressing this hemagglutinin .
	manualset3
105104	6	401628	13	NULL	NULL	0	NULL	hemagglutinin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolates expressing MR/K hemagglutinin bound in higher numbers to catheter material ( P = .023 ) than did those not expressing this hemagglutinin .
	manualset3
105105	1	401629	13	NULL	NULL	0	NULL	Isolates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolates with toxin profiles A ( + ) B ( + ) CDT ( - ) , A ( + ) B ( + ) CDT ( + ) , A ( - ) B ( + ) CDT ( - ) , and A ( - ) B ( + ) CDT ( + ) accounted for 63 % , 34 % , 2.4 % , and 0.6 % of isolates , respectively .
	manualset3
105106	2	401629	13	NULL	NULL	0	NULL	toxin profiles	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolates with toxin profiles A ( + ) B ( + ) CDT ( - ) , A ( + ) B ( + ) CDT ( + ) , A ( - ) B ( + ) CDT ( - ) , and A ( - ) B ( + ) CDT ( + ) accounted for 63 % , 34 % , 2.4 % , and 0.6 % of isolates , respectively .
	manualset3
105107	3	401629	13	NULL	NULL	0	NULL	A ( + ) B ( + ) CDT ( - ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolates with toxin profiles A ( + ) B ( + ) CDT ( - ) , A ( + ) B ( + ) CDT ( + ) , A ( - ) B ( + ) CDT ( - ) , and A ( - ) B ( + ) CDT ( + ) accounted for 63 % , 34 % , 2.4 % , and 0.6 % of isolates , respectively .
	manualset3
105108	4	401629	13	NULL	NULL	0	NULL	A ( + ) B ( + ) CDT ( + ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolates with toxin profiles A ( + ) B ( + ) CDT ( - ) , A ( + ) B ( + ) CDT ( + ) , A ( - ) B ( + ) CDT ( - ) , and A ( - ) B ( + ) CDT ( + ) accounted for 63 % , 34 % , 2.4 % , and 0.6 % of isolates , respectively .
	manualset3
105109	5	401629	13	NULL	NULL	0	NULL	A ( - ) B ( + ) CDT ( - )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolates with toxin profiles A ( + ) B ( + ) CDT ( - ) , A ( + ) B ( + ) CDT ( + ) , A ( - ) B ( + ) CDT ( - ) , and A ( - ) B ( + ) CDT ( + ) accounted for 63 % , 34 % , 2.4 % , and 0.6 % of isolates , respectively .
	manualset3
105110	6	401629	13	NULL	NULL	0	NULL	A ( - ) B ( + ) CDT ( + ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolates with toxin profiles A ( + ) B ( + ) CDT ( - ) , A ( + ) B ( + ) CDT ( + ) , A ( - ) B ( + ) CDT ( - ) , and A ( - ) B ( + ) CDT ( + ) accounted for 63 % , 34 % , 2.4 % , and 0.6 % of isolates , respectively .
	manualset3
105111	7	401629	13	NULL	NULL	0	NULL	63 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolates with toxin profiles A ( + ) B ( + ) CDT ( - ) , A ( + ) B ( + ) CDT ( + ) , A ( - ) B ( + ) CDT ( - ) , and A ( - ) B ( + ) CDT ( + ) accounted for 63 % , 34 % , 2.4 % , and 0.6 % of isolates , respectively .
	manualset3
105112	8	401629	13	NULL	NULL	0	NULL	34 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolates with toxin profiles A ( + ) B ( + ) CDT ( - ) , A ( + ) B ( + ) CDT ( + ) , A ( - ) B ( + ) CDT ( - ) , and A ( - ) B ( + ) CDT ( + ) accounted for 63 % , 34 % , 2.4 % , and 0.6 % of isolates , respectively .
	manualset3
105113	9	401629	13	NULL	NULL	0	NULL	2.4 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolates with toxin profiles A ( + ) B ( + ) CDT ( - ) , A ( + ) B ( + ) CDT ( + ) , A ( - ) B ( + ) CDT ( - ) , and A ( - ) B ( + ) CDT ( + ) accounted for 63 % , 34 % , 2.4 % , and 0.6 % of isolates , respectively .
	manualset3
105114	10	401629	13	NULL	NULL	0	NULL	0.6 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolates with toxin profiles A ( + ) B ( + ) CDT ( - ) , A ( + ) B ( + ) CDT ( + ) , A ( - ) B ( + ) CDT ( - ) , and A ( - ) B ( + ) CDT ( + ) accounted for 63 % , 34 % , 2.4 % , and 0.6 % of isolates , respectively .
	manualset3
105115	11	401629	13	NULL	NULL	0	NULL	isolates 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolates with toxin profiles A ( + ) B ( + ) CDT ( - ) , A ( + ) B ( + ) CDT ( + ) , A ( - ) B ( + ) CDT ( - ) , and A ( - ) B ( + ) CDT ( + ) accounted for 63 % , 34 % , 2.4 % , and 0.6 % of isolates , respectively .
	manualset3
105116	1	401630	13	NULL	NULL	0	NULL	Isolation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation , cloning , mapping , and nucleotide sequencing of the gene encoding flavodoxin in Escherichia coli .
	manualset3
105117	2	401630	13	NULL	NULL	0	NULL	cloning	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation , cloning , mapping , and nucleotide sequencing of the gene encoding flavodoxin in Escherichia coli .
	manualset3
105118	3	401630	13	NULL	NULL	0	NULL	mapping	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation , cloning , mapping , and nucleotide sequencing of the gene encoding flavodoxin in Escherichia coli .
	manualset3
105119	4	401630	13	NULL	NULL	0	NULL	nucleotide sequencing 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation , cloning , mapping , and nucleotide sequencing of the gene encoding flavodoxin in Escherichia coli .
	manualset3
105120	5	401630	13	NULL	NULL	NULL	NULL	gene encoding flavodoxin	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Isolation , cloning , mapping , and nucleotide sequencing of the gene encoding flavodoxin in Escherichia coli .
	manualset3
105121	6	401630	13	NULL	NULL	0	NULL	Escherichia coli 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation , cloning , mapping , and nucleotide sequencing of the gene encoding flavodoxin in Escherichia coli .
	manualset3
105122	1	401631	13	NULL	NULL	0	NULL	Isolation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation and characterization of Morris hepatoma variants unable to convert ornithine to arginine , and modulation of urea-cycle enzymes by dexamethasone and cyclic-AMP .
	manualset3
105123	2	401631	13	NULL	NULL	0	NULL	 characterization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation and characterization of Morris hepatoma variants unable to convert ornithine to arginine , and modulation of urea-cycle enzymes by dexamethasone and cyclic-AMP .
	manualset3
105124	3	401631	13	NULL	NULL	0	NULL	Morris hepatoma variants	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation and characterization of Morris hepatoma variants unable to convert ornithine to arginine , and modulation of urea-cycle enzymes by dexamethasone and cyclic-AMP .
	manualset3
105125	4	401631	13	NULL	NULL	0	NULL	ornithine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation and characterization of Morris hepatoma variants unable to convert ornithine to arginine , and modulation of urea-cycle enzymes by dexamethasone and cyclic-AMP .
	manualset3
105126	5	401631	13	NULL	NULL	0	NULL	arginine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation and characterization of Morris hepatoma variants unable to convert ornithine to arginine , and modulation of urea-cycle enzymes by dexamethasone and cyclic-AMP .
	manualset3
105127	6	401631	13	NULL	NULL	0	NULL	modulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation and characterization of Morris hepatoma variants unable to convert ornithine to arginine , and modulation of urea-cycle enzymes by dexamethasone and cyclic-AMP .
	manualset3
105128	7	401631	13	NULL	NULL	0	NULL	urea-cycle enzymes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation and characterization of Morris hepatoma variants unable to convert ornithine to arginine , and modulation of urea-cycle enzymes by dexamethasone and cyclic-AMP .
	manualset3
105129	8	401631	13	NULL	NULL	0	NULL	dexamethasone 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation and characterization of Morris hepatoma variants unable to convert ornithine to arginine , and modulation of urea-cycle enzymes by dexamethasone and cyclic-AMP .
	manualset3
105130	9	401631	13	NULL	NULL	0	NULL	cyclic-AMP 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation and characterization of Morris hepatoma variants unable to convert ornithine to arginine , and modulation of urea-cycle enzymes by dexamethasone and cyclic-AMP .
	manualset3
105131	1	401632	13	NULL	NULL	0	NULL	Isolation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation and characterization of a pea catalase cDNA .
	manualset3
105132	2	401632	13	NULL	NULL	0	NULL	characterization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation and characterization of a pea catalase cDNA .
	manualset3
105133	3	401632	13	NULL	NULL	0	NULL	pea catalase cDNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation and characterization of a pea catalase cDNA .
	manualset3
105134	1	401633	13	NULL	NULL	0	NULL	Isolation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation and characterization of microsatellite markers in the Serra Spanish mackerel , Scomberomorus brasiliensis .
	manualset3
105135	2	401633	13	NULL	NULL	0	NULL	 characterization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation and characterization of microsatellite markers in the Serra Spanish mackerel , Scomberomorus brasiliensis .
	manualset3
105136	3	401633	13	NULL	NULL	0	NULL	microsatellite markers 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation and characterization of microsatellite markers in the Serra Spanish mackerel , Scomberomorus brasiliensis .
	manualset3
105137	4	401633	13	NULL	NULL	0	NULL	Serra Spanish mackerel	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation and characterization of microsatellite markers in the Serra Spanish mackerel , Scomberomorus brasiliensis .
	manualset3
105138	5	401633	13	NULL	NULL	0	NULL	 Scomberomorus brasiliensis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation and characterization of microsatellite markers in the Serra Spanish mackerel , Scomberomorus brasiliensis .
	manualset3
105139	1	401634	13	NULL	NULL	0	NULL	Isolation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation and pharmacological characterization of a phospholipase A2 myotoxin from the venom of the Irian Jayan death adder ( Acanthophis rugosus ) .
	manualset3
105140	2	401634	13	NULL	NULL	0	NULL	pharmacological characterization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation and pharmacological characterization of a phospholipase A2 myotoxin from the venom of the Irian Jayan death adder ( Acanthophis rugosus ) .
	manualset3
105141	3	401634	13	NULL	NULL	0	NULL	phospholipase A2 myotoxin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation and pharmacological characterization of a phospholipase A2 myotoxin from the venom of the Irian Jayan death adder ( Acanthophis rugosus ) .
	manualset3
105142	4	401634	13	NULL	NULL	0	NULL	venom 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation and pharmacological characterization of a phospholipase A2 myotoxin from the venom of the Irian Jayan death adder ( Acanthophis rugosus ) .
	manualset3
105143	5	401634	13	NULL	NULL	0	NULL	Irian Jayan death adder	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation and pharmacological characterization of a phospholipase A2 myotoxin from the venom of the Irian Jayan death adder ( Acanthophis rugosus ) .
	manualset3
105144	6	401634	13	NULL	NULL	0	NULL	Acanthophis rugosus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation and pharmacological characterization of a phospholipase A2 myotoxin from the venom of the Irian Jayan death adder ( Acanthophis rugosus ) .
	manualset3
105145	1	401635	13	NULL	NULL	0	NULL	Isolation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of Leptospira by culture has a low sensitivity and the microscopic agglutination test ( MAT ) is time consuming To overcome these problems , a rapid latex agglutination test ( LAT ) has been standardized for the detection of antileptospiral antibodies in serum samples from suspected cases of leptospirosis .
	manualset3
105146	2	401635	13	NULL	NULL	0	NULL	 Leptospira	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of Leptospira by culture has a low sensitivity and the microscopic agglutination test ( MAT ) is time consuming To overcome these problems , a rapid latex agglutination test ( LAT ) has been standardized for the detection of antileptospiral antibodies in serum samples from suspected cases of leptospirosis .
	manualset3
105147	3	401635	13	NULL	NULL	0	NULL	culture	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of Leptospira by culture has a low sensitivity and the microscopic agglutination test ( MAT ) is time consuming To overcome these problems , a rapid latex agglutination test ( LAT ) has been standardized for the detection of antileptospiral antibodies in serum samples from suspected cases of leptospirosis .
	manualset3
105148	4	401635	13	NULL	NULL	0	NULL	low sensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of Leptospira by culture has a low sensitivity and the microscopic agglutination test ( MAT ) is time consuming To overcome these problems , a rapid latex agglutination test ( LAT ) has been standardized for the detection of antileptospiral antibodies in serum samples from suspected cases of leptospirosis .
	manualset3
105149	5	401635	13	NULL	NULL	0	NULL	microscopic agglutination test ( MAT ) 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of Leptospira by culture has a low sensitivity and the microscopic agglutination test ( MAT ) is time consuming To overcome these problems , a rapid latex agglutination test ( LAT ) has been standardized for the detection of antileptospiral antibodies in serum samples from suspected cases of leptospirosis .
	manualset3
105150	6	401635	13	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of Leptospira by culture has a low sensitivity and the microscopic agglutination test ( MAT ) is time consuming To overcome these problems , a rapid latex agglutination test ( LAT ) has been standardized for the detection of antileptospiral antibodies in serum samples from suspected cases of leptospirosis .
	manualset3
105151	7	401635	13	NULL	NULL	0	NULL	problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of Leptospira by culture has a low sensitivity and the microscopic agglutination test ( MAT ) is time consuming To overcome these problems , a rapid latex agglutination test ( LAT ) has been standardized for the detection of antileptospiral antibodies in serum samples from suspected cases of leptospirosis .
	manualset3
105152	8	401635	13	NULL	NULL	0	NULL	latex agglutination test ( LAT )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of Leptospira by culture has a low sensitivity and the microscopic agglutination test ( MAT ) is time consuming To overcome these problems , a rapid latex agglutination test ( LAT ) has been standardized for the detection of antileptospiral antibodies in serum samples from suspected cases of leptospirosis .
	manualset3
105153	9	401635	13	NULL	NULL	NULL	NULL	detection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Isolation of Leptospira by culture has a low sensitivity and the microscopic agglutination test ( MAT ) is time consuming To overcome these problems , a rapid latex agglutination test ( LAT ) has been standardized for the detection of antileptospiral antibodies in serum samples from suspected cases of leptospirosis .
	manualset3
105154	10	401635	13	NULL	NULL	0	NULL	 antileptospiral antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of Leptospira by culture has a low sensitivity and the microscopic agglutination test ( MAT ) is time consuming To overcome these problems , a rapid latex agglutination test ( LAT ) has been standardized for the detection of antileptospiral antibodies in serum samples from suspected cases of leptospirosis .
	manualset3
105155	11	401635	13	NULL	NULL	0	NULL	serum samples 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of Leptospira by culture has a low sensitivity and the microscopic agglutination test ( MAT ) is time consuming To overcome these problems , a rapid latex agglutination test ( LAT ) has been standardized for the detection of antileptospiral antibodies in serum samples from suspected cases of leptospirosis .
	manualset3
105156	12	401635	13	NULL	NULL	0	NULL	 cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of Leptospira by culture has a low sensitivity and the microscopic agglutination test ( MAT ) is time consuming To overcome these problems , a rapid latex agglutination test ( LAT ) has been standardized for the detection of antileptospiral antibodies in serum samples from suspected cases of leptospirosis .
	manualset3
105157	13	401635	13	NULL	NULL	0	NULL	leptospirosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of Leptospira by culture has a low sensitivity and the microscopic agglutination test ( MAT ) is time consuming To overcome these problems , a rapid latex agglutination test ( LAT ) has been standardized for the detection of antileptospiral antibodies in serum samples from suspected cases of leptospirosis .
	manualset3
105158	1	401636	13	NULL	NULL	0	NULL	Isolation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of SPINK6 in human skin : selective inhibitor of kallikrein-related peptidases .
	manualset3
105159	2	401636	13	NULL	NULL	0	NULL	 SPINK6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of SPINK6 in human skin : selective inhibitor of kallikrein-related peptidases .
	manualset3
105160	3	401636	13	NULL	NULL	0	NULL	human skin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of SPINK6 in human skin : selective inhibitor of kallikrein-related peptidases .
	manualset3
105161	4	401636	13	NULL	NULL	0	NULL	selective inhibitor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of SPINK6 in human skin : selective inhibitor of kallikrein-related peptidases .
	manualset3
105162	5	401636	13	NULL	NULL	0	NULL	kallikrein-related peptidases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of SPINK6 in human skin : selective inhibitor of kallikrein-related peptidases .
	manualset3
105163	1	401637	13	NULL	NULL	0	NULL	Isolation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of a dnaE mutation which enhances RecA-independent homologous recombination in the Escherichia coli chromosome .
	manualset3
105164	2	401637	13	NULL	NULL	0	NULL	dnaE mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of a dnaE mutation which enhances RecA-independent homologous recombination in the Escherichia coli chromosome .
	manualset3
105165	3	401637	13	NULL	NULL	0	NULL	RecA-independent homologous recombination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of a dnaE mutation which enhances RecA-independent homologous recombination in the Escherichia coli chromosome .
	manualset3
105166	4	401637	13	NULL	NULL	0	NULL	Escherichia coli chromosome	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of a dnaE mutation which enhances RecA-independent homologous recombination in the Escherichia coli chromosome .
	manualset3
105167	1	401638	13	NULL	NULL	0	NULL	Isolation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of a fluorophore-specific DNA aptamer with weak redox activity .
	manualset3
105168	2	401638	13	NULL	NULL	0	NULL	fluorophore-specific DNA aptamer 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of a fluorophore-specific DNA aptamer with weak redox activity .
	manualset3
105169	3	401638	13	NULL	NULL	0	NULL	weak redox activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of a fluorophore-specific DNA aptamer with weak redox activity .
	manualset3
105170	1	401639	13	NULL	NULL	0	NULL	Isolation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of cloned ribosomal protein genes from the yeast Saccharomyces carlsbergensis .
	manualset3
105171	2	401639	13	NULL	NULL	0	NULL	ribosomal protein genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of cloned ribosomal protein genes from the yeast Saccharomyces carlsbergensis .
	manualset3
105172	3	401639	13	NULL	NULL	0	NULL	 yeast Saccharomyces carlsbergensis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of cloned ribosomal protein genes from the yeast Saccharomyces carlsbergensis .
	manualset3
105173	1	401640	13	NULL	NULL	0	NULL	Atopic neurodermatitis -- therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Atopic neurodermatitis -- therapy in high altitude climate ) .
	manualset3
105174	2	401640	13	NULL	NULL	0	NULL	high altitude climate	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	( Atopic neurodermatitis -- therapy in high altitude climate ) .
	manualset3
105175	1	401641	13	NULL	NULL	NULL	NULL	4H7 treatments	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	4H7 treatments significantly increase osteoblast markers including alkaline phosphatase ( ALP ) , and osteocalcin ( OC ) after day 7 and day 14 of the inducing hMSCs differentiation .
	manualset3
105176	2	401641	13	NULL	NULL	0	NULL	osteoblast markers	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	4H7 treatments significantly increase osteoblast markers including alkaline phosphatase ( ALP ) , and osteocalcin ( OC ) after day 7 and day 14 of the inducing hMSCs differentiation .
	manualset3
105177	3	401641	13	NULL	NULL	0	NULL	alkaline phosphatase ( ALP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	4H7 treatments significantly increase osteoblast markers including alkaline phosphatase ( ALP ) , and osteocalcin ( OC ) after day 7 and day 14 of the inducing hMSCs differentiation .
	manualset3
105178	4	401641	13	NULL	NULL	0	NULL	osteocalcin ( OC )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	4H7 treatments significantly increase osteoblast markers including alkaline phosphatase ( ALP ) , and osteocalcin ( OC ) after day 7 and day 14 of the inducing hMSCs differentiation .
	manualset3
105179	5	401641	13	NULL	NULL	0	NULL	day 7 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	4H7 treatments significantly increase osteoblast markers including alkaline phosphatase ( ALP ) , and osteocalcin ( OC ) after day 7 and day 14 of the inducing hMSCs differentiation .
	manualset3
105180	6	401641	13	NULL	NULL	0	NULL	day 14 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	4H7 treatments significantly increase osteoblast markers including alkaline phosphatase ( ALP ) , and osteocalcin ( OC ) after day 7 and day 14 of the inducing hMSCs differentiation .
	manualset3
105181	7	401641	13	NULL	NULL	0	NULL	 hMSCs differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	4H7 treatments significantly increase osteoblast markers including alkaline phosphatase ( ALP ) , and osteocalcin ( OC ) after day 7 and day 14 of the inducing hMSCs differentiation .
	manualset3
105182	1	401642	13	NULL	NULL	0	NULL	Isolation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of mycoplasma species from the lower respiratory tract of healthy cattle and cattle with respiratory disease in Belgium .
	manualset3
105183	2	401642	13	NULL	NULL	0	NULL	mycoplasma species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of mycoplasma species from the lower respiratory tract of healthy cattle and cattle with respiratory disease in Belgium .
	manualset3
105184	3	401642	13	NULL	NULL	0	NULL	lower respiratory tract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of mycoplasma species from the lower respiratory tract of healthy cattle and cattle with respiratory disease in Belgium .
	manualset3
105185	4	401642	13	NULL	NULL	0	NULL	healthy cattle	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of mycoplasma species from the lower respiratory tract of healthy cattle and cattle with respiratory disease in Belgium .
	manualset3
105186	5	401642	13	NULL	NULL	0	NULL	cattle with respiratory disease	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of mycoplasma species from the lower respiratory tract of healthy cattle and cattle with respiratory disease in Belgium .
	manualset3
105187	6	401642	13	NULL	NULL	0	NULL	Belgium 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of mycoplasma species from the lower respiratory tract of healthy cattle and cattle with respiratory disease in Belgium .
	manualset3
105188	1	401643	13	NULL	NULL	0	NULL	Isolation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of ribosomes from the cell walls of barley ( Hordeum vulgare ) .
	manualset3
105189	2	401643	13	NULL	NULL	0	NULL	ribosomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of ribosomes from the cell walls of barley ( Hordeum vulgare ) .
	manualset3
105190	3	401643	13	NULL	NULL	0	NULL	cell walls	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of ribosomes from the cell walls of barley ( Hordeum vulgare ) .
	manualset3
105191	4	401643	13	NULL	NULL	0	NULL	barley	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of ribosomes from the cell walls of barley ( Hordeum vulgare ) .
	manualset3
105192	5	401643	13	NULL	NULL	0	NULL	Hordeum vulgare 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of ribosomes from the cell walls of barley ( Hordeum vulgare ) .
	manualset3
105193	1	401644	13	NULL	NULL	0	NULL	Isolation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of the fluorescent hydrolysis product from acid hydrolyzates of oligo - and polydeoxyribonucleotides has shown that the photoadduct is formed by ultraviolet irradiation of d ( pTpA ) , d ( TpApT ) , d ( TpApTpA ) , poly ( dA-dT ) , and both single - and double-stranded DNA .
	manualset3
105194	2	401644	13	NULL	NULL	0	NULL	fluorescent hydrolysis product 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of the fluorescent hydrolysis product from acid hydrolyzates of oligo - and polydeoxyribonucleotides has shown that the photoadduct is formed by ultraviolet irradiation of d ( pTpA ) , d ( TpApT ) , d ( TpApTpA ) , poly ( dA-dT ) , and both single - and double-stranded DNA .
	manualset3
105195	3	401644	13	NULL	NULL	0	NULL	acid hydrolyzates of oligodeoxyribonucleotides	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of the fluorescent hydrolysis product from acid hydrolyzates of oligo - and polydeoxyribonucleotides has shown that the photoadduct is formed by ultraviolet irradiation of d ( pTpA ) , d ( TpApT ) , d ( TpApTpA ) , poly ( dA-dT ) , and both single - and double-stranded DNA .
	manualset3
105196	4	401644	13	NULL	NULL	0	NULL	acid hydrolyzates of  polydeoxyribonucleotides	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of the fluorescent hydrolysis product from acid hydrolyzates of oligo - and polydeoxyribonucleotides has shown that the photoadduct is formed by ultraviolet irradiation of d ( pTpA ) , d ( TpApT ) , d ( TpApTpA ) , poly ( dA-dT ) , and both single - and double-stranded DNA .
	manualset3
105197	5	401644	13	NULL	NULL	0	NULL	photoadduct	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of the fluorescent hydrolysis product from acid hydrolyzates of oligo - and polydeoxyribonucleotides has shown that the photoadduct is formed by ultraviolet irradiation of d ( pTpA ) , d ( TpApT ) , d ( TpApTpA ) , poly ( dA-dT ) , and both single - and double-stranded DNA .
	manualset3
105198	6	401644	13	NULL	NULL	0	NULL	ultraviolet irradiation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of the fluorescent hydrolysis product from acid hydrolyzates of oligo - and polydeoxyribonucleotides has shown that the photoadduct is formed by ultraviolet irradiation of d ( pTpA ) , d ( TpApT ) , d ( TpApTpA ) , poly ( dA-dT ) , and both single - and double-stranded DNA .
	manualset3
105199	7	401644	13	NULL	NULL	0	NULL	d ( pTpA ) 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of the fluorescent hydrolysis product from acid hydrolyzates of oligo - and polydeoxyribonucleotides has shown that the photoadduct is formed by ultraviolet irradiation of d ( pTpA ) , d ( TpApT ) , d ( TpApTpA ) , poly ( dA-dT ) , and both single - and double-stranded DNA .
	manualset3
105200	8	401644	13	NULL	NULL	0	NULL	d ( TpApT )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of the fluorescent hydrolysis product from acid hydrolyzates of oligo - and polydeoxyribonucleotides has shown that the photoadduct is formed by ultraviolet irradiation of d ( pTpA ) , d ( TpApT ) , d ( TpApTpA ) , poly ( dA-dT ) , and both single - and double-stranded DNA .
	manualset3
105201	9	401644	13	NULL	NULL	0	NULL	d ( TpApTpA ) 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of the fluorescent hydrolysis product from acid hydrolyzates of oligo - and polydeoxyribonucleotides has shown that the photoadduct is formed by ultraviolet irradiation of d ( pTpA ) , d ( TpApT ) , d ( TpApTpA ) , poly ( dA-dT ) , and both single - and double-stranded DNA .
	manualset3
105202	10	401644	13	NULL	NULL	0	NULL	poly ( dA-dT )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of the fluorescent hydrolysis product from acid hydrolyzates of oligo - and polydeoxyribonucleotides has shown that the photoadduct is formed by ultraviolet irradiation of d ( pTpA ) , d ( TpApT ) , d ( TpApTpA ) , poly ( dA-dT ) , and both single - and double-stranded DNA .
	manualset3
105203	11	401644	13	NULL	NULL	0	NULL	single-stranded DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of the fluorescent hydrolysis product from acid hydrolyzates of oligo - and polydeoxyribonucleotides has shown that the photoadduct is formed by ultraviolet irradiation of d ( pTpA ) , d ( TpApT ) , d ( TpApTpA ) , poly ( dA-dT ) , and both single - and double-stranded DNA .
	manualset3
105204	12	401644	13	NULL	NULL	0	NULL	double-stranded DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of the fluorescent hydrolysis product from acid hydrolyzates of oligo - and polydeoxyribonucleotides has shown that the photoadduct is formed by ultraviolet irradiation of d ( pTpA ) , d ( TpApT ) , d ( TpApTpA ) , poly ( dA-dT ) , and both single - and double-stranded DNA .
	manualset3
105205	1	401645	13	NULL	NULL	0	NULL	Isolation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of two cytochrome P450 forms , CYP2A19 and CYP1A , from pig liver microsomes .
	manualset3
105206	2	401645	13	NULL	NULL	0	NULL	 two cytochrome P450 forms	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of two cytochrome P450 forms , CYP2A19 and CYP1A , from pig liver microsomes .
	manualset3
105207	3	401645	13	NULL	NULL	0	NULL	CYP2A19	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of two cytochrome P450 forms , CYP2A19 and CYP1A , from pig liver microsomes .
	manualset3
105208	4	401645	13	NULL	NULL	0	NULL	CYP1A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of two cytochrome P450 forms , CYP2A19 and CYP1A , from pig liver microsomes .
	manualset3
105209	5	401645	13	NULL	NULL	0	NULL	pig liver microsomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of two cytochrome P450 forms , CYP2A19 and CYP1A , from pig liver microsomes .
	manualset3
105210	1	401646	13	NULL	NULL	0	NULL	Isolation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of zebrafish gdf7 and comparative genetic mapping of genes belonging to the growth/differentiation factor 5 , 6 , 7 subgroup of the TGF-beta superfamily .
	manualset3
105211	2	401646	13	NULL	NULL	NULL	NULL	zebrafish gdf7 	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Isolation of zebrafish gdf7 and comparative genetic mapping of genes belonging to the growth/differentiation factor 5 , 6 , 7 subgroup of the TGF-beta superfamily .
	manualset3
105212	3	401646	13	NULL	NULL	0	NULL	comparative genetic mapping	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of zebrafish gdf7 and comparative genetic mapping of genes belonging to the growth/differentiation factor 5 , 6 , 7 subgroup of the TGF-beta superfamily .
	manualset3
105213	4	401646	13	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of zebrafish gdf7 and comparative genetic mapping of genes belonging to the growth/differentiation factor 5 , 6 , 7 subgroup of the TGF-beta superfamily .
	manualset3
105214	5	401646	13	NULL	NULL	0	NULL	growth/differentiation factor 5 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of zebrafish gdf7 and comparative genetic mapping of genes belonging to the growth/differentiation factor 5 , 6 , 7 subgroup of the TGF-beta superfamily .
	manualset3
105215	6	401646	13	NULL	NULL	0	NULL	growth/differentiation factor 6	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of zebrafish gdf7 and comparative genetic mapping of genes belonging to the growth/differentiation factor 5 , 6 , 7 subgroup of the TGF-beta superfamily .
	manualset3
105216	7	401646	13	NULL	NULL	NULL	NULL	growth/differentiation factor 7	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Isolation of zebrafish gdf7 and comparative genetic mapping of genes belonging to the growth/differentiation factor 5 , 6 , 7 subgroup of the TGF-beta superfamily .
	manualset3
105217	8	401646	13	NULL	NULL	0	NULL	subgroup of the TGF-beta superfamily	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of zebrafish gdf7 and comparative genetic mapping of genes belonging to the growth/differentiation factor 5 , 6 , 7 subgroup of the TGF-beta superfamily .
	manualset3
105218	1	401647	13	NULL	NULL	0	NULL	Isolation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation to interface to integration - is it feasible to seek a holistic profession ?
	manualset3
105219	2	401647	13	NULL	NULL	0	NULL	 interface	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation to interface to integration - is it feasible to seek a holistic profession ?
	manualset3
105220	3	401647	13	NULL	NULL	0	NULL	integration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation to interface to integration - is it feasible to seek a holistic profession ?
	manualset3
105221	4	401647	13	NULL	NULL	0	NULL	holistic profession	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation to interface to integration - is it feasible to seek a holistic profession ?
	manualset3
105222	1	401648	13	NULL	NULL	0	NULL	Isoleucine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Isoleucine , threonine , phenylalanine , and summation .
	manualset3
105223	2	401648	13	NULL	NULL	0	NULL	threonine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Isoleucine , threonine , phenylalanine , and summation .
	manualset3
105224	3	401648	13	NULL	NULL	0	NULL	phenylalanine 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Isoleucine , threonine , phenylalanine , and summation .
	manualset3
105225	4	401648	13	NULL	NULL	0	NULL	summation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Isoleucine , threonine , phenylalanine , and summation .
	manualset3
105226	1	401649	13	NULL	NULL	0	NULL	Isoproterenol stimulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Isoproterenol stimulation of adenylate cyclase activity is lost completely in ureters from 90 day and older animals .
	manualset3
105227	2	401649	13	NULL	NULL	0	NULL	adenylate cyclase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Isoproterenol stimulation of adenylate cyclase activity is lost completely in ureters from 90 day and older animals .
	manualset3
105228	3	401649	13	NULL	NULL	0	NULL	ureters	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Isoproterenol stimulation of adenylate cyclase activity is lost completely in ureters from 90 day and older animals .
	manualset3
105229	4	401649	13	NULL	NULL	0	NULL	90 day animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Isoproterenol stimulation of adenylate cyclase activity is lost completely in ureters from 90 day and older animals .
	manualset3
105230	5	401649	13	NULL	NULL	0	NULL	older animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Isoproterenol stimulation of adenylate cyclase activity is lost completely in ureters from 90 day and older animals .
	manualset3
105231	1	401650	13	NULL	NULL	0	NULL	5-HT ( 2C ) receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	5-HT ( 2C ) receptors are transiently expressed in a patchy fashion in the visual cortex of kittens between 30-80 days of age complementary to patches demarcated by cytochrome oxidase staining .
	manualset3
105232	2	401650	13	NULL	NULL	0	NULL	patchy fashion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	5-HT ( 2C ) receptors are transiently expressed in a patchy fashion in the visual cortex of kittens between 30-80 days of age complementary to patches demarcated by cytochrome oxidase staining .
	manualset3
105233	3	401650	13	NULL	NULL	0	NULL	visual cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	5-HT ( 2C ) receptors are transiently expressed in a patchy fashion in the visual cortex of kittens between 30-80 days of age complementary to patches demarcated by cytochrome oxidase staining .
	manualset3
105234	4	401650	13	NULL	NULL	0	NULL	kittens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	5-HT ( 2C ) receptors are transiently expressed in a patchy fashion in the visual cortex of kittens between 30-80 days of age complementary to patches demarcated by cytochrome oxidase staining .
	manualset3
105235	5	401650	13	NULL	NULL	0	NULL	30-80 days of age 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	5-HT ( 2C ) receptors are transiently expressed in a patchy fashion in the visual cortex of kittens between 30-80 days of age complementary to patches demarcated by cytochrome oxidase staining .
	manualset3
105236	6	401650	13	NULL	NULL	NULL	NULL	patches 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	5-HT ( 2C ) receptors are transiently expressed in a patchy fashion in the visual cortex of kittens between 30-80 days of age complementary to patches demarcated by cytochrome oxidase staining .
	manualset3
105237	7	401650	13	NULL	NULL	0	NULL	cytochrome oxidase staining 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	5-HT ( 2C ) receptors are transiently expressed in a patchy fashion in the visual cortex of kittens between 30-80 days of age complementary to patches demarcated by cytochrome oxidase staining .
	manualset3
105238	1	401651	13	NULL	NULL	0	NULL	Isovolumic rabbit hearts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Isovolumic rabbit hearts ( n = 7 ) were perfused retrogradely with hemoglobin-free Tyrode solution at 37 degrees C. Coronary venous O2 tension was measured polarographically , and tissue oxygenation was measured with two-wavelength near-infrared spectroscopy ( NIRS ) , both at a time resolution of approximately 2 s. During transitions to anoxia , 68 + / - 2 % ( SE ) of the NIRS signal was due to Mb and the rest to cytochrome oxidase .
	manualset3
105239	2	401651	13	NULL	NULL	0	NULL	n = 7	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Isovolumic rabbit hearts ( n = 7 ) were perfused retrogradely with hemoglobin-free Tyrode solution at 37 degrees C. Coronary venous O2 tension was measured polarographically , and tissue oxygenation was measured with two-wavelength near-infrared spectroscopy ( NIRS ) , both at a time resolution of approximately 2 s. During transitions to anoxia , 68 + / - 2 % ( SE ) of the NIRS signal was due to Mb and the rest to cytochrome oxidase .
	manualset3
105240	3	401651	13	NULL	NULL	0	NULL	hemoglobin-free Tyrode solution 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Isovolumic rabbit hearts ( n = 7 ) were perfused retrogradely with hemoglobin-free Tyrode solution at 37 degrees C. Coronary venous O2 tension was measured polarographically , and tissue oxygenation was measured with two-wavelength near-infrared spectroscopy ( NIRS ) , both at a time resolution of approximately 2 s. During transitions to anoxia , 68 + / - 2 % ( SE ) of the NIRS signal was due to Mb and the rest to cytochrome oxidase .
	manualset3
105241	4	401651	13	NULL	NULL	0	NULL	37 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Isovolumic rabbit hearts ( n = 7 ) were perfused retrogradely with hemoglobin-free Tyrode solution at 37 degrees C. Coronary venous O2 tension was measured polarographically , and tissue oxygenation was measured with two-wavelength near-infrared spectroscopy ( NIRS ) , both at a time resolution of approximately 2 s. During transitions to anoxia , 68 + / - 2 % ( SE ) of the NIRS signal was due to Mb and the rest to cytochrome oxidase .
	manualset3
105242	5	401651	13	NULL	NULL	0	NULL	Coronary venous O2 tension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Isovolumic rabbit hearts ( n = 7 ) were perfused retrogradely with hemoglobin-free Tyrode solution at 37 degrees C. Coronary venous O2 tension was measured polarographically , and tissue oxygenation was measured with two-wavelength near-infrared spectroscopy ( NIRS ) , both at a time resolution of approximately 2 s. During transitions to anoxia , 68 + / - 2 % ( SE ) of the NIRS signal was due to Mb and the rest to cytochrome oxidase .
	manualset3
105243	6	401651	13	NULL	NULL	0	NULL	tissue oxygenation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Isovolumic rabbit hearts ( n = 7 ) were perfused retrogradely with hemoglobin-free Tyrode solution at 37 degrees C. Coronary venous O2 tension was measured polarographically , and tissue oxygenation was measured with two-wavelength near-infrared spectroscopy ( NIRS ) , both at a time resolution of approximately 2 s. During transitions to anoxia , 68 + / - 2 % ( SE ) of the NIRS signal was due to Mb and the rest to cytochrome oxidase .
	manualset3
105244	7	401651	13	NULL	NULL	0	NULL	two-wavelength near-infrared spectroscopy ( NIRS )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Isovolumic rabbit hearts ( n = 7 ) were perfused retrogradely with hemoglobin-free Tyrode solution at 37 degrees C. Coronary venous O2 tension was measured polarographically , and tissue oxygenation was measured with two-wavelength near-infrared spectroscopy ( NIRS ) , both at a time resolution of approximately 2 s. During transitions to anoxia , 68 + / - 2 % ( SE ) of the NIRS signal was due to Mb and the rest to cytochrome oxidase .
	manualset3
105245	8	401651	13	NULL	NULL	0	NULL	time resolution	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Isovolumic rabbit hearts ( n = 7 ) were perfused retrogradely with hemoglobin-free Tyrode solution at 37 degrees C. Coronary venous O2 tension was measured polarographically , and tissue oxygenation was measured with two-wavelength near-infrared spectroscopy ( NIRS ) , both at a time resolution of approximately 2 s. During transitions to anoxia , 68 + / - 2 % ( SE ) of the NIRS signal was due to Mb and the rest to cytochrome oxidase .
	manualset3
105246	9	401651	13	NULL	NULL	0	NULL	approximately 2 s	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Isovolumic rabbit hearts ( n = 7 ) were perfused retrogradely with hemoglobin-free Tyrode solution at 37 degrees C. Coronary venous O2 tension was measured polarographically , and tissue oxygenation was measured with two-wavelength near-infrared spectroscopy ( NIRS ) , both at a time resolution of approximately 2 s. During transitions to anoxia , 68 + / - 2 % ( SE ) of the NIRS signal was due to Mb and the rest to cytochrome oxidase .
	manualset3
105247	10	401651	13	NULL	NULL	0	NULL	transitions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Isovolumic rabbit hearts ( n = 7 ) were perfused retrogradely with hemoglobin-free Tyrode solution at 37 degrees C. Coronary venous O2 tension was measured polarographically , and tissue oxygenation was measured with two-wavelength near-infrared spectroscopy ( NIRS ) , both at a time resolution of approximately 2 s. During transitions to anoxia , 68 + / - 2 % ( SE ) of the NIRS signal was due to Mb and the rest to cytochrome oxidase .
	manualset3
105248	11	401651	13	NULL	NULL	0	NULL	anoxia	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Isovolumic rabbit hearts ( n = 7 ) were perfused retrogradely with hemoglobin-free Tyrode solution at 37 degrees C. Coronary venous O2 tension was measured polarographically , and tissue oxygenation was measured with two-wavelength near-infrared spectroscopy ( NIRS ) , both at a time resolution of approximately 2 s. During transitions to anoxia , 68 + / - 2 % ( SE ) of the NIRS signal was due to Mb and the rest to cytochrome oxidase .
	manualset3
105249	12	401651	13	NULL	NULL	0	NULL	68 + / - 2 % ( SE ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Isovolumic rabbit hearts ( n = 7 ) were perfused retrogradely with hemoglobin-free Tyrode solution at 37 degrees C. Coronary venous O2 tension was measured polarographically , and tissue oxygenation was measured with two-wavelength near-infrared spectroscopy ( NIRS ) , both at a time resolution of approximately 2 s. During transitions to anoxia , 68 + / - 2 % ( SE ) of the NIRS signal was due to Mb and the rest to cytochrome oxidase .
	manualset3
105250	13	401651	13	NULL	NULL	0	NULL	NIRS signal	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Isovolumic rabbit hearts ( n = 7 ) were perfused retrogradely with hemoglobin-free Tyrode solution at 37 degrees C. Coronary venous O2 tension was measured polarographically , and tissue oxygenation was measured with two-wavelength near-infrared spectroscopy ( NIRS ) , both at a time resolution of approximately 2 s. During transitions to anoxia , 68 + / - 2 % ( SE ) of the NIRS signal was due to Mb and the rest to cytochrome oxidase .
	manualset3
105251	14	401651	13	NULL	NULL	0	NULL	Mb 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Isovolumic rabbit hearts ( n = 7 ) were perfused retrogradely with hemoglobin-free Tyrode solution at 37 degrees C. Coronary venous O2 tension was measured polarographically , and tissue oxygenation was measured with two-wavelength near-infrared spectroscopy ( NIRS ) , both at a time resolution of approximately 2 s. During transitions to anoxia , 68 + / - 2 % ( SE ) of the NIRS signal was due to Mb and the rest to cytochrome oxidase .
	manualset3
105252	15	401651	13	NULL	NULL	0	NULL	cytochrome oxidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Isovolumic rabbit hearts ( n = 7 ) were perfused retrogradely with hemoglobin-free Tyrode solution at 37 degrees C. Coronary venous O2 tension was measured polarographically , and tissue oxygenation was measured with two-wavelength near-infrared spectroscopy ( NIRS ) , both at a time resolution of approximately 2 s. During transitions to anoxia , 68 + / - 2 % ( SE ) of the NIRS signal was due to Mb and the rest to cytochrome oxidase .
	manualset3
105253	1	401652	13	NULL	NULL	0	NULL	Issues	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Issues addressed included the facilitator 's outlook towards PBL , previous experiences which helped to make a smoother transition into their teaching position , approaches that assisted in preparing faculty and students to teach and learn in a PBL program , academic resources referenced by faculty members , and the use of nonclinical tutors in a physician assistant PBL program .
	manualset3
105254	2	401652	13	NULL	NULL	0	NULL	facilitator 's 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Issues addressed included the facilitator 's outlook towards PBL , previous experiences which helped to make a smoother transition into their teaching position , approaches that assisted in preparing faculty and students to teach and learn in a PBL program , academic resources referenced by faculty members , and the use of nonclinical tutors in a physician assistant PBL program .
	manualset3
105255	3	401652	13	NULL	NULL	0	NULL	outlook	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Issues addressed included the facilitator 's outlook towards PBL , previous experiences which helped to make a smoother transition into their teaching position , approaches that assisted in preparing faculty and students to teach and learn in a PBL program , academic resources referenced by faculty members , and the use of nonclinical tutors in a physician assistant PBL program .
	manualset3
105256	4	401652	13	NULL	NULL	0	NULL	PBL	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Issues addressed included the facilitator 's outlook towards PBL , previous experiences which helped to make a smoother transition into their teaching position , approaches that assisted in preparing faculty and students to teach and learn in a PBL program , academic resources referenced by faculty members , and the use of nonclinical tutors in a physician assistant PBL program .
	manualset3
105257	5	401652	13	NULL	NULL	0	NULL	previous experiences	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Issues addressed included the facilitator 's outlook towards PBL , previous experiences which helped to make a smoother transition into their teaching position , approaches that assisted in preparing faculty and students to teach and learn in a PBL program , academic resources referenced by faculty members , and the use of nonclinical tutors in a physician assistant PBL program .
	manualset3
105258	6	401652	13	NULL	NULL	0	NULL	smoother transition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Issues addressed included the facilitator 's outlook towards PBL , previous experiences which helped to make a smoother transition into their teaching position , approaches that assisted in preparing faculty and students to teach and learn in a PBL program , academic resources referenced by faculty members , and the use of nonclinical tutors in a physician assistant PBL program .
	manualset3
105259	7	401652	13	NULL	NULL	0	NULL	 teaching position	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Issues addressed included the facilitator 's outlook towards PBL , previous experiences which helped to make a smoother transition into their teaching position , approaches that assisted in preparing faculty and students to teach and learn in a PBL program , academic resources referenced by faculty members , and the use of nonclinical tutors in a physician assistant PBL program .
	manualset3
105260	8	401652	13	NULL	NULL	0	NULL	approaches	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Issues addressed included the facilitator 's outlook towards PBL , previous experiences which helped to make a smoother transition into their teaching position , approaches that assisted in preparing faculty and students to teach and learn in a PBL program , academic resources referenced by faculty members , and the use of nonclinical tutors in a physician assistant PBL program .
	manualset3
105261	9	401652	13	NULL	NULL	NULL	NULL	faculty	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Issues addressed included the facilitator 's outlook towards PBL , previous experiences which helped to make a smoother transition into their teaching position , approaches that assisted in preparing faculty and students to teach and learn in a PBL program , academic resources referenced by faculty members , and the use of nonclinical tutors in a physician assistant PBL program .
	manualset3
105262	10	401652	13	NULL	NULL	0	NULL	students	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Issues addressed included the facilitator 's outlook towards PBL , previous experiences which helped to make a smoother transition into their teaching position , approaches that assisted in preparing faculty and students to teach and learn in a PBL program , academic resources referenced by faculty members , and the use of nonclinical tutors in a physician assistant PBL program .
	manualset3
105265	13	401652	13	NULL	NULL	0	NULL	PBL program	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Issues addressed included the facilitator 's outlook towards PBL , previous experiences which helped to make a smoother transition into their teaching position , approaches that assisted in preparing faculty and students to teach and learn in a PBL program , academic resources referenced by faculty members , and the use of nonclinical tutors in a physician assistant PBL program .
	manualset3
105266	14	401652	13	NULL	NULL	NULL	NULL	academic resources 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Issues addressed included the facilitator 's outlook towards PBL , previous experiences which helped to make a smoother transition into their teaching position , approaches that assisted in preparing faculty and students to teach and learn in a PBL program , academic resources referenced by faculty members , and the use of nonclinical tutors in a physician assistant PBL program .
	manualset3
105267	15	401652	13	NULL	NULL	0	NULL	faculty members	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Issues addressed included the facilitator 's outlook towards PBL , previous experiences which helped to make a smoother transition into their teaching position , approaches that assisted in preparing faculty and students to teach and learn in a PBL program , academic resources referenced by faculty members , and the use of nonclinical tutors in a physician assistant PBL program .
	manualset3
105268	16	401652	13	NULL	NULL	0	NULL	use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Issues addressed included the facilitator 's outlook towards PBL , previous experiences which helped to make a smoother transition into their teaching position , approaches that assisted in preparing faculty and students to teach and learn in a PBL program , academic resources referenced by faculty members , and the use of nonclinical tutors in a physician assistant PBL program .
	manualset3
105269	17	401652	13	NULL	NULL	0	NULL	nonclinical tutors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Issues addressed included the facilitator 's outlook towards PBL , previous experiences which helped to make a smoother transition into their teaching position , approaches that assisted in preparing faculty and students to teach and learn in a PBL program , academic resources referenced by faculty members , and the use of nonclinical tutors in a physician assistant PBL program .
	manualset3
105270	18	401652	13	NULL	NULL	0	NULL	physician assistant PBL program	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Issues addressed included the facilitator 's outlook towards PBL , previous experiences which helped to make a smoother transition into their teaching position , approaches that assisted in preparing faculty and students to teach and learn in a PBL program , academic resources referenced by faculty members , and the use of nonclinical tutors in a physician assistant PBL program .
	manualset3
105271	1	401653	13	NULL	NULL	0	NULL	approximately 5 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It accounts for approximately 5 % of all thyroid cancers .
	manualset3
105272	2	401653	13	NULL	NULL	0	NULL	thyroid cancers	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It accounts for approximately 5 % of all thyroid cancers .
	manualset3
105273	1	401654	13	NULL	NULL	0	NULL	 8 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It affects 8 % of the adult population and is associated with significant morbidity and increased risk to individual and society .
	manualset3
105274	2	401654	13	NULL	NULL	0	NULL	 adult population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It affects 8 % of the adult population and is associated with significant morbidity and increased risk to individual and society .
	manualset3
105275	3	401654	13	NULL	NULL	0	NULL	 morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It affects 8 % of the adult population and is associated with significant morbidity and increased risk to individual and society .
	manualset3
105276	4	401654	13	NULL	NULL	0	NULL	risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It affects 8 % of the adult population and is associated with significant morbidity and increased risk to individual and society .
	manualset3
105277	5	401654	13	NULL	NULL	0	NULL	individual	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	It affects 8 % of the adult population and is associated with significant morbidity and increased risk to individual and society .
	manualset3
105278	6	401654	13	NULL	NULL	0	NULL	society	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It affects 8 % of the adult population and is associated with significant morbidity and increased risk to individual and society .
	manualset3
105279	1	401655	13	NULL	NULL	0	NULL	temporal changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It aims to observe temporal changes in local epidermal thickness and oxyhemoglobin concentration and to gain insight into the progression of foot ulcer formation and healing .
	manualset3
105280	2	401655	13	NULL	NULL	0	NULL	local epidermal thickness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It aims to observe temporal changes in local epidermal thickness and oxyhemoglobin concentration and to gain insight into the progression of foot ulcer formation and healing .
	manualset3
105281	3	401655	13	NULL	NULL	0	NULL	oxyhemoglobin concentration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It aims to observe temporal changes in local epidermal thickness and oxyhemoglobin concentration and to gain insight into the progression of foot ulcer formation and healing .
	manualset3
105282	4	401655	13	NULL	NULL	NULL	NULL	insight	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It aims to observe temporal changes in local epidermal thickness and oxyhemoglobin concentration and to gain insight into the progression of foot ulcer formation and healing .
	manualset3
105283	5	401655	13	NULL	NULL	0	NULL	progression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It aims to observe temporal changes in local epidermal thickness and oxyhemoglobin concentration and to gain insight into the progression of foot ulcer formation and healing .
	manualset3
105284	6	401655	13	NULL	NULL	0	NULL	foot ulcer formation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It aims to observe temporal changes in local epidermal thickness and oxyhemoglobin concentration and to gain insight into the progression of foot ulcer formation and healing .
	manualset3
105285	7	401655	13	NULL	NULL	0	NULL	healing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It aims to observe temporal changes in local epidermal thickness and oxyhemoglobin concentration and to gain insight into the progression of foot ulcer formation and healing .
	manualset3
105286	1	401656	13	NULL	NULL	0	NULL	5-HT2 sites	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	5-HT2 sites , labeled by ( 125I ) 7-amino-8-iodo ketanserin , were decreased in parietal cerebral cortex layers 3 and 5 by imipramine treatment , but not by tianeptine treatment and not by daily restraint stress .
	manualset3
105287	2	401656	13	NULL	NULL	0	NULL	( 125I ) 7-amino-8-iodo ketanserin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	5-HT2 sites , labeled by ( 125I ) 7-amino-8-iodo ketanserin , were decreased in parietal cerebral cortex layers 3 and 5 by imipramine treatment , but not by tianeptine treatment and not by daily restraint stress .
	manualset3
105288	3	401656	13	NULL	NULL	0	NULL	parietal cerebral cortex layers 3	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	5-HT2 sites , labeled by ( 125I ) 7-amino-8-iodo ketanserin , were decreased in parietal cerebral cortex layers 3 and 5 by imipramine treatment , but not by tianeptine treatment and not by daily restraint stress .
	manualset3
105289	4	401656	13	NULL	NULL	0	NULL	parietal cerebral cortex layers 5	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	5-HT2 sites , labeled by ( 125I ) 7-amino-8-iodo ketanserin , were decreased in parietal cerebral cortex layers 3 and 5 by imipramine treatment , but not by tianeptine treatment and not by daily restraint stress .
	manualset3
105290	5	401656	13	NULL	NULL	0	NULL	imipramine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	5-HT2 sites , labeled by ( 125I ) 7-amino-8-iodo ketanserin , were decreased in parietal cerebral cortex layers 3 and 5 by imipramine treatment , but not by tianeptine treatment and not by daily restraint stress .
	manualset3
105291	6	401656	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	5-HT2 sites , labeled by ( 125I ) 7-amino-8-iodo ketanserin , were decreased in parietal cerebral cortex layers 3 and 5 by imipramine treatment , but not by tianeptine treatment and not by daily restraint stress .
	manualset3
105292	7	401656	13	NULL	NULL	0	NULL	tianeptine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	5-HT2 sites , labeled by ( 125I ) 7-amino-8-iodo ketanserin , were decreased in parietal cerebral cortex layers 3 and 5 by imipramine treatment , but not by tianeptine treatment and not by daily restraint stress .
	manualset3
105293	8	401656	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	5-HT2 sites , labeled by ( 125I ) 7-amino-8-iodo ketanserin , were decreased in parietal cerebral cortex layers 3 and 5 by imipramine treatment , but not by tianeptine treatment and not by daily restraint stress .
	manualset3
105294	9	401656	13	NULL	NULL	0	NULL	daily restraint stress 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	5-HT2 sites , labeled by ( 125I ) 7-amino-8-iodo ketanserin , were decreased in parietal cerebral cortex layers 3 and 5 by imipramine treatment , but not by tianeptine treatment and not by daily restraint stress .
	manualset3
105295	1	401657	13	NULL	NULL	0	NULL	planners	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It allows planners to vary their assumptions , such as the biological agent used , treatment efficacy , and speed of providing initial treatment .
	manualset3
105296	2	401657	13	NULL	NULL	0	NULL	assumptions	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It allows planners to vary their assumptions , such as the biological agent used , treatment efficacy , and speed of providing initial treatment .
	manualset3
105297	3	401657	13	NULL	NULL	0	NULL	biological agent	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It allows planners to vary their assumptions , such as the biological agent used , treatment efficacy , and speed of providing initial treatment .
	manualset3
105298	4	401657	13	NULL	NULL	0	NULL	treatment efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It allows planners to vary their assumptions , such as the biological agent used , treatment efficacy , and speed of providing initial treatment .
	manualset3
105299	5	401657	13	NULL	NULL	0	NULL	speed	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It allows planners to vary their assumptions , such as the biological agent used , treatment efficacy , and speed of providing initial treatment .
	manualset3
105300	6	401657	13	NULL	NULL	0	NULL	initial treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It allows planners to vary their assumptions , such as the biological agent used , treatment efficacy , and speed of providing initial treatment .
	manualset3
105301	1	401658	13	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It allows women to choose birth intervals and family size freely .
	manualset3
105302	2	401658	13	NULL	NULL	0	NULL	birth intervals	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	It allows women to choose birth intervals and family size freely .
	manualset3
105303	3	401658	13	NULL	NULL	0	NULL	family size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It allows women to choose birth intervals and family size freely .
	manualset3
105304	1	401659	13	NULL	NULL	0	NULL	increase in temperature 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It also decreased with an increase in temperature , whereas the breakthrough time of the MB canister did not change with temperature .
	manualset3
105305	2	401659	13	NULL	NULL	0	NULL	breakthrough time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	It also decreased with an increase in temperature , whereas the breakthrough time of the MB canister did not change with temperature .
	manualset3
105306	3	401659	13	NULL	NULL	0	NULL	MB canister 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It also decreased with an increase in temperature , whereas the breakthrough time of the MB canister did not change with temperature .
	manualset3
105307	4	401659	13	NULL	NULL	0	NULL	temperature	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	It also decreased with an increase in temperature , whereas the breakthrough time of the MB canister did not change with temperature .
	manualset3
105308	1	401660	13	NULL	NULL	0	NULL	 bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It also facilitates the bacteria growing and the potein producing obviously .
	manualset3
105310	3	401660	13	NULL	NULL	0	NULL	potein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It also facilitates the bacteria growing and the potein producing obviously .
	manualset3
105311	1	401661	13	NULL	NULL	0	NULL	covalent protein-DNA complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It also forms a covalent protein-DNA complex with negatively supercoiled DNA in the absence of Mg2 + but requires Mg2 + for the relaxation of negatively supercoiled DNA .
	manualset3
105312	2	401661	13	NULL	NULL	NULL	NULL	negatively supercoiled DNA 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It also forms a covalent protein-DNA complex with negatively supercoiled DNA in the absence of Mg2 + but requires Mg2 + for the relaxation of negatively supercoiled DNA .
	manualset3
105313	3	401661	13	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It also forms a covalent protein-DNA complex with negatively supercoiled DNA in the absence of Mg2 + but requires Mg2 + for the relaxation of negatively supercoiled DNA .
	manualset3
105314	4	401661	13	NULL	NULL	0	NULL	 Mg2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	It also forms a covalent protein-DNA complex with negatively supercoiled DNA in the absence of Mg2 + but requires Mg2 + for the relaxation of negatively supercoiled DNA .
	manualset3
105315	5	401661	13	NULL	NULL	0	NULL	 Mg2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	It also forms a covalent protein-DNA complex with negatively supercoiled DNA in the absence of Mg2 + but requires Mg2 + for the relaxation of negatively supercoiled DNA .
	manualset3
105316	6	401661	13	NULL	NULL	0	NULL	relaxation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It also forms a covalent protein-DNA complex with negatively supercoiled DNA in the absence of Mg2 + but requires Mg2 + for the relaxation of negatively supercoiled DNA .
	manualset3
105317	7	401661	13	NULL	NULL	0	NULL	negatively supercoiled DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It also forms a covalent protein-DNA complex with negatively supercoiled DNA in the absence of Mg2 + but requires Mg2 + for the relaxation of negatively supercoiled DNA .
	manualset3
105318	1	401662	13	NULL	NULL	0	NULL	palliative care team	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It also helps a palliative care team decide which , among many potential opportunities and possible initiatives , is the one most likely to be supported by the institution and have a recognized and significant impact .
	manualset3
105319	2	401662	13	NULL	NULL	0	NULL	opportunities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It also helps a palliative care team decide which , among many potential opportunities and possible initiatives , is the one most likely to be supported by the institution and have a recognized and significant impact .
	manualset3
105320	3	401662	13	NULL	NULL	0	NULL	initiatives	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It also helps a palliative care team decide which , among many potential opportunities and possible initiatives , is the one most likely to be supported by the institution and have a recognized and significant impact .
	manualset3
105321	4	401662	13	NULL	NULL	0	NULL	institution	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It also helps a palliative care team decide which , among many potential opportunities and possible initiatives , is the one most likely to be supported by the institution and have a recognized and significant impact .
	manualset3
105322	5	401662	13	NULL	NULL	0	NULL	impact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It also helps a palliative care team decide which , among many potential opportunities and possible initiatives , is the one most likely to be supported by the institution and have a recognized and significant impact .
	manualset3
105323	1	401663	13	NULL	NULL	0	NULL	highlights 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It also highlights some of the key insights into filament function that have come from these studies .
	manualset3
105324	2	401663	13	NULL	NULL	0	NULL	key insights	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It also highlights some of the key insights into filament function that have come from these studies .
	manualset3
105325	3	401663	13	NULL	NULL	0	NULL	filament function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It also highlights some of the key insights into filament function that have come from these studies .
	manualset3
105326	4	401663	13	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	It also highlights some of the key insights into filament function that have come from these studies .
	manualset3
105327	1	401664	13	NULL	NULL	0	NULL	5-Hydroxytryptamine	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	5-Hydroxytryptamine injected into posterior and anterior parts of the pigeon hypothalamus evoked a short lasting hyperthermia or hypothermia , respectively .
	manualset3
105328	2	401664	13	NULL	NULL	0	NULL	posterior parts of the pigeon hypothalamus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	5-Hydroxytryptamine injected into posterior and anterior parts of the pigeon hypothalamus evoked a short lasting hyperthermia or hypothermia , respectively .
	manualset3
105329	3	401664	13	NULL	NULL	0	NULL	anterior parts of the pigeon hypothalamus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	5-Hydroxytryptamine injected into posterior and anterior parts of the pigeon hypothalamus evoked a short lasting hyperthermia or hypothermia , respectively .
	manualset3
105330	4	401664	13	NULL	NULL	0	NULL	hyperthermia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	5-Hydroxytryptamine injected into posterior and anterior parts of the pigeon hypothalamus evoked a short lasting hyperthermia or hypothermia , respectively .
	manualset3
105331	5	401664	13	NULL	NULL	0	NULL	hypothermia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	5-Hydroxytryptamine injected into posterior and anterior parts of the pigeon hypothalamus evoked a short lasting hyperthermia or hypothermia , respectively .
	manualset3
105332	1	401665	13	NULL	NULL	0	NULL	bronchial responsiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It also increases bronchial responsiveness and causes airway sensitization to several occupational allergens .
	manualset3
105333	2	401665	13	NULL	NULL	0	NULL	causes airway sensitization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It also increases bronchial responsiveness and causes airway sensitization to several occupational allergens .
	manualset3
105334	3	401665	13	NULL	NULL	0	NULL	occupational allergens	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It also increases bronchial responsiveness and causes airway sensitization to several occupational allergens .
	manualset3
105335	1	401666	13	NULL	NULL	0	NULL	oxygen uptake rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It also means that the overall oxygen uptake rate for A. oryzae is much higher than the oxygen uptake rate that can be predicted in the densely packed mycelium layer for R. oligosporus and C. minitans .
	manualset3
105336	2	401666	13	NULL	NULL	0	NULL	A. oryzae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It also means that the overall oxygen uptake rate for A. oryzae is much higher than the oxygen uptake rate that can be predicted in the densely packed mycelium layer for R. oligosporus and C. minitans .
	manualset3
105337	3	401666	13	NULL	NULL	0	NULL	oxygen uptake rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It also means that the overall oxygen uptake rate for A. oryzae is much higher than the oxygen uptake rate that can be predicted in the densely packed mycelium layer for R. oligosporus and C. minitans .
	manualset3
105338	4	401666	13	NULL	NULL	0	NULL	mycelium layer	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It also means that the overall oxygen uptake rate for A. oryzae is much higher than the oxygen uptake rate that can be predicted in the densely packed mycelium layer for R. oligosporus and C. minitans .
	manualset3
105339	5	401666	13	NULL	NULL	0	NULL	R. oligosporus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It also means that the overall oxygen uptake rate for A. oryzae is much higher than the oxygen uptake rate that can be predicted in the densely packed mycelium layer for R. oligosporus and C. minitans .
	manualset3
105340	6	401666	13	NULL	NULL	NULL	NULL	C. minitans	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It also means that the overall oxygen uptake rate for A. oryzae is much higher than the oxygen uptake rate that can be predicted in the densely packed mycelium layer for R. oligosporus and C. minitans .
	manualset3
105341	1	401667	13	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	It also provides further evidence for the efficacy of this innovative assessment method in which standardized and validated psychometric tests are formatted for computer presentation and simultaneous recording of neural activity , which serves as the response measure in lieu of verbal/behavioral responses .
	manualset3
105342	2	401667	13	NULL	NULL	0	NULL	efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It also provides further evidence for the efficacy of this innovative assessment method in which standardized and validated psychometric tests are formatted for computer presentation and simultaneous recording of neural activity , which serves as the response measure in lieu of verbal/behavioral responses .
	manualset3
105343	3	401667	13	NULL	NULL	0	NULL	 innovative assessment method 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It also provides further evidence for the efficacy of this innovative assessment method in which standardized and validated psychometric tests are formatted for computer presentation and simultaneous recording of neural activity , which serves as the response measure in lieu of verbal/behavioral responses .
	manualset3
105344	4	401667	13	NULL	NULL	0	NULL	psychometric tests	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It also provides further evidence for the efficacy of this innovative assessment method in which standardized and validated psychometric tests are formatted for computer presentation and simultaneous recording of neural activity , which serves as the response measure in lieu of verbal/behavioral responses .
	manualset3
105345	5	401667	13	NULL	NULL	0	NULL	computer presentation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It also provides further evidence for the efficacy of this innovative assessment method in which standardized and validated psychometric tests are formatted for computer presentation and simultaneous recording of neural activity , which serves as the response measure in lieu of verbal/behavioral responses .
	manualset3
105346	6	401667	13	NULL	NULL	0	NULL	recording	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It also provides further evidence for the efficacy of this innovative assessment method in which standardized and validated psychometric tests are formatted for computer presentation and simultaneous recording of neural activity , which serves as the response measure in lieu of verbal/behavioral responses .
	manualset3
105347	7	401667	13	NULL	NULL	0	NULL	neural activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It also provides further evidence for the efficacy of this innovative assessment method in which standardized and validated psychometric tests are formatted for computer presentation and simultaneous recording of neural activity , which serves as the response measure in lieu of verbal/behavioral responses .
	manualset3
105348	8	401667	13	NULL	NULL	0	NULL	response measure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It also provides further evidence for the efficacy of this innovative assessment method in which standardized and validated psychometric tests are formatted for computer presentation and simultaneous recording of neural activity , which serves as the response measure in lieu of verbal/behavioral responses .
	manualset3
105349	9	401667	13	NULL	NULL	0	NULL	verbal/behavioral responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It also provides further evidence for the efficacy of this innovative assessment method in which standardized and validated psychometric tests are formatted for computer presentation and simultaneous recording of neural activity , which serves as the response measure in lieu of verbal/behavioral responses .
	manualset3
105350	1	401668	13	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	It also provides the first evidence that glucans can directly modulate the functional activity of NHDF .
	manualset3
105351	2	401668	13	NULL	NULL	0	NULL	 glucans	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It also provides the first evidence that glucans can directly modulate the functional activity of NHDF .
	manualset3
105352	3	401668	13	NULL	NULL	0	NULL	functional activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It also provides the first evidence that glucans can directly modulate the functional activity of NHDF .
	manualset3
105353	4	401668	13	NULL	NULL	0	NULL	NHDF	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It also provides the first evidence that glucans can directly modulate the functional activity of NHDF .
	manualset3
105354	1	401669	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It also show that cells considered as less active can still act as resources for phages , although they contain much less intracellular phage particles .
	manualset3
105355	2	401669	13	NULL	NULL	0	NULL	resources	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It also show that cells considered as less active can still act as resources for phages , although they contain much less intracellular phage particles .
	manualset3
105356	3	401669	13	NULL	NULL	0	NULL	phages	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It also show that cells considered as less active can still act as resources for phages , although they contain much less intracellular phage particles .
	manualset3
105357	4	401669	13	NULL	NULL	NULL	NULL	intracellular phage particles 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It also show that cells considered as less active can still act as resources for phages , although they contain much less intracellular phage particles .
	manualset3
105358	1	401670	13	NULL	NULL	0	NULL	SMC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It appeared that SMC hyperplasia in the intima contributed more often to a reduction of luminal patency than medial hyalinosis in allylamine-fed rats .
	manualset3
105359	2	401670	13	NULL	NULL	0	NULL	hyperplasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It appeared that SMC hyperplasia in the intima contributed more often to a reduction of luminal patency than medial hyalinosis in allylamine-fed rats .
	manualset3
105360	3	401670	13	NULL	NULL	0	NULL	intima	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It appeared that SMC hyperplasia in the intima contributed more often to a reduction of luminal patency than medial hyalinosis in allylamine-fed rats .
	manualset3
105361	4	401670	13	NULL	NULL	0	NULL	reduction of luminal patency 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It appeared that SMC hyperplasia in the intima contributed more often to a reduction of luminal patency than medial hyalinosis in allylamine-fed rats .
	manualset3
105362	5	401670	13	NULL	NULL	0	NULL	medial hyalinosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It appeared that SMC hyperplasia in the intima contributed more often to a reduction of luminal patency than medial hyalinosis in allylamine-fed rats .
	manualset3
105363	6	401670	13	NULL	NULL	0	NULL	allylamine-fed rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It appeared that SMC hyperplasia in the intima contributed more often to a reduction of luminal patency than medial hyalinosis in allylamine-fed rats .
	manualset3
105364	1	401671	13	NULL	NULL	0	NULL	 defensin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It appears as though defensin is stored in the granulocytes of the hemolymph and secreted into the hemolymph upon bacterial insult .
	manualset3
105365	2	401671	13	NULL	NULL	0	NULL	granulocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It appears as though defensin is stored in the granulocytes of the hemolymph and secreted into the hemolymph upon bacterial insult .
	manualset3
105366	3	401671	13	NULL	NULL	0	NULL	hemolymph	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It appears as though defensin is stored in the granulocytes of the hemolymph and secreted into the hemolymph upon bacterial insult .
	manualset3
105367	4	401671	13	NULL	NULL	0	NULL	hemolymph	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It appears as though defensin is stored in the granulocytes of the hemolymph and secreted into the hemolymph upon bacterial insult .
	manualset3
105368	5	401671	13	NULL	NULL	0	NULL	bacterial insult	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It appears as though defensin is stored in the granulocytes of the hemolymph and secreted into the hemolymph upon bacterial insult .
	manualset3
105369	1	401672	13	NULL	NULL	0	NULL	neural transmission	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It appears that neural transmission is impaired by either direct disruption of dopaminergic transmission or a more general impairment of neurotransmission that gives rise to compensatory changes in monoaminergic systems that are not sufficient to completely normalize neural function .
	manualset3
105370	2	401672	13	NULL	NULL	0	NULL	disruption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It appears that neural transmission is impaired by either direct disruption of dopaminergic transmission or a more general impairment of neurotransmission that gives rise to compensatory changes in monoaminergic systems that are not sufficient to completely normalize neural function .
	manualset3
105371	3	401672	13	NULL	NULL	0	NULL	dopaminergic transmission	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It appears that neural transmission is impaired by either direct disruption of dopaminergic transmission or a more general impairment of neurotransmission that gives rise to compensatory changes in monoaminergic systems that are not sufficient to completely normalize neural function .
	manualset3
105372	4	401672	13	NULL	NULL	0	NULL	general impairment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It appears that neural transmission is impaired by either direct disruption of dopaminergic transmission or a more general impairment of neurotransmission that gives rise to compensatory changes in monoaminergic systems that are not sufficient to completely normalize neural function .
	manualset3
105373	5	401672	13	NULL	NULL	0	NULL	neurotransmission 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It appears that neural transmission is impaired by either direct disruption of dopaminergic transmission or a more general impairment of neurotransmission that gives rise to compensatory changes in monoaminergic systems that are not sufficient to completely normalize neural function .
	manualset3
105374	6	401672	13	NULL	NULL	NULL	NULL	gives rise to	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It appears that neural transmission is impaired by either direct disruption of dopaminergic transmission or a more general impairment of neurotransmission that gives rise to compensatory changes in monoaminergic systems that are not sufficient to completely normalize neural function .
	manualset3
105375	7	401672	13	NULL	NULL	0	NULL	compensatory changes 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It appears that neural transmission is impaired by either direct disruption of dopaminergic transmission or a more general impairment of neurotransmission that gives rise to compensatory changes in monoaminergic systems that are not sufficient to completely normalize neural function .
	manualset3
105376	8	401672	13	NULL	NULL	0	NULL	monoaminergic systems	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It appears that neural transmission is impaired by either direct disruption of dopaminergic transmission or a more general impairment of neurotransmission that gives rise to compensatory changes in monoaminergic systems that are not sufficient to completely normalize neural function .
	manualset3
105377	9	401672	13	NULL	NULL	0	NULL	neural function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It appears that neural transmission is impaired by either direct disruption of dopaminergic transmission or a more general impairment of neurotransmission that gives rise to compensatory changes in monoaminergic systems that are not sufficient to completely normalize neural function .
	manualset3
105378	1	401673	13	NULL	NULL	0	NULL	 lipid binding domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	It appears then that the lipid binding domain of the pancreatic lipase protein cofactor comprises two regions .
	manualset3
105379	2	401673	13	NULL	NULL	0	NULL	pancreatic lipase protein cofactor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It appears then that the lipid binding domain of the pancreatic lipase protein cofactor comprises two regions .
	manualset3
105380	3	401673	13	NULL	NULL	0	NULL	two regions	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	It appears then that the lipid binding domain of the pancreatic lipase protein cofactor comprises two regions .
	manualset3
105381	1	401674	13	NULL	NULL	0	NULL	 continuum model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	It assumes an underlining continuum model , in which the total amount of mass is exactly preserved during the transformation of tissues .
	manualset3
105382	2	401674	13	NULL	NULL	0	NULL	 total amount of mass	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It assumes an underlining continuum model , in which the total amount of mass is exactly preserved during the transformation of tissues .
	manualset3
105383	3	401674	13	NULL	NULL	0	NULL	transformation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It assumes an underlining continuum model , in which the total amount of mass is exactly preserved during the transformation of tissues .
	manualset3
105384	4	401674	13	NULL	NULL	0	NULL	tissues 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	It assumes an underlining continuum model , in which the total amount of mass is exactly preserved during the transformation of tissues .
	manualset3
105385	1	401675	13	NULL	NULL	0	NULL	diagnostic importance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It assumes diagnostic importance when found in association with various vascular conditions ; when found in association with a characteristic symptomatology , it may be used to support a diagnosis of latent tetany .
	manualset3
105386	2	401675	13	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	It assumes diagnostic importance when found in association with various vascular conditions ; when found in association with a characteristic symptomatology , it may be used to support a diagnosis of latent tetany .
	manualset3
105387	3	401675	13	NULL	NULL	0	NULL	vascular conditions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It assumes diagnostic importance when found in association with various vascular conditions ; when found in association with a characteristic symptomatology , it may be used to support a diagnosis of latent tetany .
	manualset3
105388	4	401675	13	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	It assumes diagnostic importance when found in association with various vascular conditions ; when found in association with a characteristic symptomatology , it may be used to support a diagnosis of latent tetany .
	manualset3
105389	5	401675	13	NULL	NULL	0	NULL	characteristic symptomatology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It assumes diagnostic importance when found in association with various vascular conditions ; when found in association with a characteristic symptomatology , it may be used to support a diagnosis of latent tetany .
	manualset3
105390	6	401675	13	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It assumes diagnostic importance when found in association with various vascular conditions ; when found in association with a characteristic symptomatology , it may be used to support a diagnosis of latent tetany .
	manualset3
105391	7	401675	13	NULL	NULL	0	NULL	 latent tetany	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It assumes diagnostic importance when found in association with various vascular conditions ; when found in association with a characteristic symptomatology , it may be used to support a diagnosis of latent tetany .
	manualset3
105392	1	401676	13	NULL	NULL	0	NULL	 links 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	It begins by analyzing the close links between food and employment in the development process .
	manualset3
105393	2	401676	13	NULL	NULL	0	NULL	food 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	It begins by analyzing the close links between food and employment in the development process .
	manualset3
105394	3	401676	13	NULL	NULL	0	NULL	 employment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It begins by analyzing the close links between food and employment in the development process .
	manualset3
105395	4	401676	13	NULL	NULL	0	NULL	development process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It begins by analyzing the close links between food and employment in the development process .
	manualset3
105396	1	401677	13	NULL	NULL	0	NULL	fatty acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It binds fatty acids stoichiometrically in a 1 : 1 ratio .
	manualset3
105397	2	401677	13	NULL	NULL	0	NULL	1 : 1 ratio 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It binds fatty acids stoichiometrically in a 1 : 1 ratio .
	manualset3
105399	2	401678	13	NULL	NULL	0	NULL	HIV fusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It blocks HIV fusion to host cells .
	manualset3
105400	3	401678	13	NULL	NULL	0	NULL	host cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It blocks HIV fusion to host cells .
	manualset3
105401	1	401679	13	NULL	NULL	0	NULL	 use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It can be concluded that the use of meniscal allografts in clinical practice has progressed to a point where relief of pain may be expected for the short-term .
	manualset3
105402	2	401679	13	NULL	NULL	0	NULL	meniscal allografts	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	It can be concluded that the use of meniscal allografts in clinical practice has progressed to a point where relief of pain may be expected for the short-term .
	manualset3
105403	3	401679	13	NULL	NULL	0	NULL	clinical practice 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It can be concluded that the use of meniscal allografts in clinical practice has progressed to a point where relief of pain may be expected for the short-term .
	manualset3
105404	4	401679	13	NULL	NULL	0	NULL	point	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It can be concluded that the use of meniscal allografts in clinical practice has progressed to a point where relief of pain may be expected for the short-term .
	manualset3
105405	5	401679	13	NULL	NULL	0	NULL	relief of pain 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It can be concluded that the use of meniscal allografts in clinical practice has progressed to a point where relief of pain may be expected for the short-term .
	manualset3
105406	1	401680	13	NULL	NULL	0	NULL	invasion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It can be performed without further invasion in conjunction with cystometry .
	manualset3
105407	2	401680	13	NULL	NULL	0	NULL	conjunction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It can be performed without further invasion in conjunction with cystometry .
	manualset3
105408	3	401680	13	NULL	NULL	0	NULL	cystometry 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It can be performed without further invasion in conjunction with cystometry .
	manualset3
105409	1	401681	13	NULL	NULL	0	NULL	 antioxidants 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It can be reduced by antioxidants such as selenium , melatonin , and the selective nNOS inhibitor , 7-nitroindazole .
	manualset3
105410	2	401681	13	NULL	NULL	0	NULL	selenium 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	It can be reduced by antioxidants such as selenium , melatonin , and the selective nNOS inhibitor , 7-nitroindazole .
	manualset3
105411	3	401681	13	NULL	NULL	0	NULL	melatonin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It can be reduced by antioxidants such as selenium , melatonin , and the selective nNOS inhibitor , 7-nitroindazole .
	manualset3
105412	4	401681	13	NULL	NULL	0	NULL	selective nNOS inhibitor 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	It can be reduced by antioxidants such as selenium , melatonin , and the selective nNOS inhibitor , 7-nitroindazole .
	manualset3
105413	5	401681	13	NULL	NULL	0	NULL	7-nitroindazole	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	It can be reduced by antioxidants such as selenium , melatonin , and the selective nNOS inhibitor , 7-nitroindazole .
	manualset3
105414	1	401682	13	NULL	NULL	0	NULL	cleavage 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It can be speculated that the cleavage of CLEC3A by MMP-7 weakens the stable adhesion of tumor cells to the matrix and promotes their migration in tumor microenvironments .
	manualset3
105415	2	401682	13	NULL	NULL	0	NULL	 CLEC3A 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It can be speculated that the cleavage of CLEC3A by MMP-7 weakens the stable adhesion of tumor cells to the matrix and promotes their migration in tumor microenvironments .
	manualset3
105416	3	401682	13	NULL	NULL	0	NULL	MMP-7	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It can be speculated that the cleavage of CLEC3A by MMP-7 weakens the stable adhesion of tumor cells to the matrix and promotes their migration in tumor microenvironments .
	manualset3
105417	4	401682	13	NULL	NULL	0	NULL	stable adhesion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It can be speculated that the cleavage of CLEC3A by MMP-7 weakens the stable adhesion of tumor cells to the matrix and promotes their migration in tumor microenvironments .
	manualset3
105418	5	401682	13	NULL	NULL	0	NULL	tumor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It can be speculated that the cleavage of CLEC3A by MMP-7 weakens the stable adhesion of tumor cells to the matrix and promotes their migration in tumor microenvironments .
	manualset3
105419	6	401682	13	NULL	NULL	0	NULL	matrix 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It can be speculated that the cleavage of CLEC3A by MMP-7 weakens the stable adhesion of tumor cells to the matrix and promotes their migration in tumor microenvironments .
	manualset3
105420	7	401682	13	NULL	NULL	0	NULL	migration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It can be speculated that the cleavage of CLEC3A by MMP-7 weakens the stable adhesion of tumor cells to the matrix and promotes their migration in tumor microenvironments .
	manualset3
105421	8	401682	13	NULL	NULL	0	NULL	 tumor microenvironments	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It can be speculated that the cleavage of CLEC3A by MMP-7 weakens the stable adhesion of tumor cells to the matrix and promotes their migration in tumor microenvironments .
	manualset3
105422	1	401683	13	NULL	NULL	0	NULL	variety of insults	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It can develop following a variety of insults but is most commonly encountered as a complication of parotidectomy .
	manualset3
105423	2	401683	13	NULL	NULL	0	NULL	complication 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It can develop following a variety of insults but is most commonly encountered as a complication of parotidectomy .
	manualset3
105424	3	401683	13	NULL	NULL	0	NULL	parotidectomy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It can develop following a variety of insults but is most commonly encountered as a complication of parotidectomy .
	manualset3
105425	1	401684	13	NULL	NULL	NULL	NULL	amassment 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It can not be ruled out that the amassment of adrenalin in the perinfraction zone may be causative of arrhythmias and recurrent lesions of the myocardium .
	manualset3
105426	2	401684	13	NULL	NULL	0	NULL	 adrenalin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It can not be ruled out that the amassment of adrenalin in the perinfraction zone may be causative of arrhythmias and recurrent lesions of the myocardium .
	manualset3
105427	3	401684	13	NULL	NULL	0	NULL	perinfraction zone	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It can not be ruled out that the amassment of adrenalin in the perinfraction zone may be causative of arrhythmias and recurrent lesions of the myocardium .
	manualset3
105428	4	401684	13	NULL	NULL	0	NULL	arrhythmias 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It can not be ruled out that the amassment of adrenalin in the perinfraction zone may be causative of arrhythmias and recurrent lesions of the myocardium .
	manualset3
105429	5	401684	13	NULL	NULL	0	NULL	recurrent lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It can not be ruled out that the amassment of adrenalin in the perinfraction zone may be causative of arrhythmias and recurrent lesions of the myocardium .
	manualset3
105430	6	401684	13	NULL	NULL	0	NULL	myocardium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It can not be ruled out that the amassment of adrenalin in the perinfraction zone may be causative of arrhythmias and recurrent lesions of the myocardium .
	manualset3
105431	1	401685	13	NULL	NULL	0	NULL	substrate	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	It can use it as a substrate that goes in and off the active site or as a cofactor to provide an electron transferase activity to the polypeptide .
	manualset3
105432	2	401685	13	NULL	NULL	0	NULL	active site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	It can use it as a substrate that goes in and off the active site or as a cofactor to provide an electron transferase activity to the polypeptide .
	manualset3
105433	3	401685	13	NULL	NULL	0	NULL	cofactor 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It can use it as a substrate that goes in and off the active site or as a cofactor to provide an electron transferase activity to the polypeptide .
	manualset3
105434	4	401685	13	NULL	NULL	0	NULL	electron transferase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It can use it as a substrate that goes in and off the active site or as a cofactor to provide an electron transferase activity to the polypeptide .
	manualset3
105435	5	401685	13	NULL	NULL	0	NULL	polypeptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	It can use it as a substrate that goes in and off the active site or as a cofactor to provide an electron transferase activity to the polypeptide .
	manualset3
105436	1	401686	13	NULL	NULL	0	NULL	unilateral tinnitus 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It caused unilateral tinnitus , facial weakness , trigeminal hypesthesia , and vertigo with lateropulsion .
	manualset3
105437	2	401686	13	NULL	NULL	0	NULL	facial weakness 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It caused unilateral tinnitus , facial weakness , trigeminal hypesthesia , and vertigo with lateropulsion .
	manualset3
105438	3	401686	13	NULL	NULL	0	NULL	trigeminal hypesthesia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It caused unilateral tinnitus , facial weakness , trigeminal hypesthesia , and vertigo with lateropulsion .
	manualset3
105439	4	401686	13	NULL	NULL	0	NULL	vertigo	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It caused unilateral tinnitus , facial weakness , trigeminal hypesthesia , and vertigo with lateropulsion .
	manualset3
105440	5	401686	13	NULL	NULL	0	NULL	lateropulsion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It caused unilateral tinnitus , facial weakness , trigeminal hypesthesia , and vertigo with lateropulsion .
	manualset3
105441	1	401687	13	NULL	NULL	0	NULL	 density	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	5 ) , corresponding to a density of 1.56 + / - 0.22 g cm ( -3 ) ( refs 2 , 5 ) .
	manualset3
105442	2	401687	13	NULL	NULL	0	NULL	1.56 + / - 0.22 g cm ( -3 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	5 ) , corresponding to a density of 1.56 + / - 0.22 g cm ( -3 ) ( refs 2 , 5 ) .
	manualset3
105443	3	401687	13	NULL	NULL	0	NULL	refs 2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	5 ) , corresponding to a density of 1.56 + / - 0.22 g cm ( -3 ) ( refs 2 , 5 ) .
	manualset3
105444	4	401687	13	NULL	NULL	0	NULL	refs 5 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	5 ) , corresponding to a density of 1.56 + / - 0.22 g cm ( -3 ) ( refs 2 , 5 ) .
	manualset3
105445	1	401688	13	NULL	NULL	0	NULL	involvement	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It confirms the involvement of mitochondria in the proapoptotic activity of NaBt .
	manualset3
105446	2	401688	13	NULL	NULL	0	NULL	mitochondria	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	It confirms the involvement of mitochondria in the proapoptotic activity of NaBt .
	manualset3
105447	3	401688	13	NULL	NULL	0	NULL	proapoptotic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It confirms the involvement of mitochondria in the proapoptotic activity of NaBt .
	manualset3
105448	4	401688	13	NULL	NULL	0	NULL	NaBt 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It confirms the involvement of mitochondria in the proapoptotic activity of NaBt .
	manualset3
105449	1	401689	13	NULL	NULL	0	NULL	 novel ( alpha alpha ) ( 7 ) barrel 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	It consists of a novel ( alpha alpha ) ( 7 ) barrel containing the active site that includes essential acidic residues and calcium .
	manualset3
105450	2	401689	13	NULL	NULL	NULL	NULL	active site 	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It consists of a novel ( alpha alpha ) ( 7 ) barrel containing the active site that includes essential acidic residues and calcium .
	manualset3
105451	3	401689	13	NULL	NULL	0	NULL	essential acidic residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It consists of a novel ( alpha alpha ) ( 7 ) barrel containing the active site that includes essential acidic residues and calcium .
	manualset3
105452	4	401689	13	NULL	NULL	0	NULL	calcium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	It consists of a novel ( alpha alpha ) ( 7 ) barrel containing the active site that includes essential acidic residues and calcium .
	manualset3
105453	1	401690	13	NULL	NULL	0	NULL	single polypeptide chain 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	It consists of a single polypeptide chain and undergoes reduction in molecular weight from 50 , 000 to 38 , 000 upon activation by proteases but not by dissociative treatment .
	manualset3
105454	2	401690	13	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It consists of a single polypeptide chain and undergoes reduction in molecular weight from 50 , 000 to 38 , 000 upon activation by proteases but not by dissociative treatment .
	manualset3
105455	3	401690	13	NULL	NULL	0	NULL	molecular weight 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It consists of a single polypeptide chain and undergoes reduction in molecular weight from 50 , 000 to 38 , 000 upon activation by proteases but not by dissociative treatment .
	manualset3
105456	4	401690	13	NULL	NULL	0	NULL	50 , 000 to 38 , 000	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It consists of a single polypeptide chain and undergoes reduction in molecular weight from 50 , 000 to 38 , 000 upon activation by proteases but not by dissociative treatment .
	manualset3
105457	5	401690	13	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It consists of a single polypeptide chain and undergoes reduction in molecular weight from 50 , 000 to 38 , 000 upon activation by proteases but not by dissociative treatment .
	manualset3
105458	6	401690	13	NULL	NULL	0	NULL	proteases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It consists of a single polypeptide chain and undergoes reduction in molecular weight from 50 , 000 to 38 , 000 upon activation by proteases but not by dissociative treatment .
	manualset3
105459	7	401690	13	NULL	NULL	0	NULL	dissociative treatment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It consists of a single polypeptide chain and undergoes reduction in molecular weight from 50 , 000 to 38 , 000 upon activation by proteases but not by dissociative treatment .
	manualset3
105460	1	401691	13	NULL	NULL	0	NULL	extracellular domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	It consists of an extracellular domain , a single transmembrane domain , and an intracellular domain .
	manualset3
105461	2	401691	13	NULL	NULL	0	NULL	single transmembrane domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	It consists of an extracellular domain , a single transmembrane domain , and an intracellular domain .
	manualset3
105462	3	401691	13	NULL	NULL	0	NULL	intracellular domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	It consists of an extracellular domain , a single transmembrane domain , and an intracellular domain .
	manualset3
105463	1	401692	13	NULL	NULL	0	NULL	works 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	It contained works by the most important authors on mathematics , astronomy , and astrology from the classical , medieval , and early modern periods .
	manualset3
105464	2	401692	13	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It contained works by the most important authors on mathematics , astronomy , and astrology from the classical , medieval , and early modern periods .
	manualset3
105465	3	401692	13	NULL	NULL	0	NULL	mathematics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	It contained works by the most important authors on mathematics , astronomy , and astrology from the classical , medieval , and early modern periods .
	manualset3
105466	4	401692	13	NULL	NULL	0	NULL	astronomy	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	It contained works by the most important authors on mathematics , astronomy , and astrology from the classical , medieval , and early modern periods .
	manualset3
105467	5	401692	13	NULL	NULL	0	NULL	astrology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	It contained works by the most important authors on mathematics , astronomy , and astrology from the classical , medieval , and early modern periods .
	manualset3
105468	6	401692	13	NULL	NULL	0	NULL	 classical periods	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	It contained works by the most important authors on mathematics , astronomy , and astrology from the classical , medieval , and early modern periods .
	manualset3
105469	7	401692	13	NULL	NULL	0	NULL	medieval periods	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	It contained works by the most important authors on mathematics , astronomy , and astrology from the classical , medieval , and early modern periods .
	manualset3
105470	8	401692	13	NULL	NULL	0	NULL	early modern periods	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	It contained works by the most important authors on mathematics , astronomy , and astrology from the classical , medieval , and early modern periods .
	manualset3
105471	1	401693	13	NULL	NULL	0	NULL	putative amino-terminal signal peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	It contains a putative amino-terminal signal peptide , basic processing sites , and a carboxyl-terminal amidation signal .
	manualset3
105472	2	401693	13	NULL	NULL	0	NULL	basic processing sites 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	It contains a putative amino-terminal signal peptide , basic processing sites , and a carboxyl-terminal amidation signal .
	manualset3
105473	3	401693	13	NULL	NULL	0	NULL	carboxyl-terminal amidation signal	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It contains a putative amino-terminal signal peptide , basic processing sites , and a carboxyl-terminal amidation signal .
	manualset3
105474	1	401694	13	NULL	NULL	0	NULL	tumor promoter	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It could be shown that the tumor promoter 12-O-tetradecanoylphorbol-13-acetate , despite initiating the release of prostaglandin E2 , had little effect on the release of leukotriene C4-like immunoreactivity .
	manualset3
105475	2	401694	13	NULL	NULL	0	NULL	12-O-tetradecanoylphorbol-13-acetate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It could be shown that the tumor promoter 12-O-tetradecanoylphorbol-13-acetate , despite initiating the release of prostaglandin E2 , had little effect on the release of leukotriene C4-like immunoreactivity .
	manualset3
105476	3	401694	13	NULL	NULL	0	NULL	release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It could be shown that the tumor promoter 12-O-tetradecanoylphorbol-13-acetate , despite initiating the release of prostaglandin E2 , had little effect on the release of leukotriene C4-like immunoreactivity .
	manualset3
105477	4	401694	13	NULL	NULL	0	NULL	prostaglandin E2	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It could be shown that the tumor promoter 12-O-tetradecanoylphorbol-13-acetate , despite initiating the release of prostaglandin E2 , had little effect on the release of leukotriene C4-like immunoreactivity .
	manualset3
105478	5	401694	13	NULL	NULL	0	NULL	effect 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It could be shown that the tumor promoter 12-O-tetradecanoylphorbol-13-acetate , despite initiating the release of prostaglandin E2 , had little effect on the release of leukotriene C4-like immunoreactivity .
	manualset3
105479	6	401694	13	NULL	NULL	NULL	NULL	release	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It could be shown that the tumor promoter 12-O-tetradecanoylphorbol-13-acetate , despite initiating the release of prostaglandin E2 , had little effect on the release of leukotriene C4-like immunoreactivity .
	manualset3
105480	7	401694	13	NULL	NULL	0	NULL	leukotriene C4-like immunoreactivity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It could be shown that the tumor promoter 12-O-tetradecanoylphorbol-13-acetate , despite initiating the release of prostaglandin E2 , had little effect on the release of leukotriene C4-like immunoreactivity .
	manualset3
105481	1	401695	13	NULL	NULL	0	NULL	5 - to 5.2-fold over the level	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	5 - to 5.2-fold over the level expected by simple addition of the 2 agents ( DMFs 3.5-5 .2 ) .
	manualset3
105482	2	401695	13	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	5 - to 5.2-fold over the level expected by simple addition of the 2 agents ( DMFs 3.5-5 .2 ) .
	manualset3
105483	3	401695	13	NULL	NULL	0	NULL	2 agents ( DMFs 3.5-5 .2 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	5 - to 5.2-fold over the level expected by simple addition of the 2 agents ( DMFs 3.5-5 .2 ) .
	manualset3
105484	1	401696	13	NULL	NULL	0	NULL	 nomifensine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	It demonstrated that nomifensine has distinct antidepressive and activating effects .
	manualset3
105485	2	401696	13	NULL	NULL	0	NULL	antidepressive effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It demonstrated that nomifensine has distinct antidepressive and activating effects .
	manualset3
105486	3	401696	13	NULL	NULL	0	NULL	activating effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It demonstrated that nomifensine has distinct antidepressive and activating effects .
	manualset3
105487	1	401697	13	NULL	NULL	NULL	NULL	right	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It denies that the right to engage in abortion is `` deeply rooted in this Nation 's history or tradition . ''
	manualset3
105488	2	401697	13	NULL	NULL	0	NULL	abortion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It denies that the right to engage in abortion is `` deeply rooted in this Nation 's history or tradition . ''
	manualset3
105489	3	401697	13	NULL	NULL	0	NULL	Nation 's history	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It denies that the right to engage in abortion is `` deeply rooted in this Nation 's history or tradition . ''
	manualset3
105490	4	401697	13	NULL	NULL	0	NULL	tradition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It denies that the right to engage in abortion is `` deeply rooted in this Nation 's history or tradition . ''
	manualset3
105491	1	401698	13	NULL	NULL	0	NULL	construction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It describes the construction of the 35-item Identity Consolidation Inventory ( ICI ) and , as an appendix to the paper , includes the final version of this questionnaire .
	manualset3
105492	2	401698	13	NULL	NULL	0	NULL	35-item 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It describes the construction of the 35-item Identity Consolidation Inventory ( ICI ) and , as an appendix to the paper , includes the final version of this questionnaire .
	manualset3
105493	3	401698	13	NULL	NULL	0	NULL	Identity Consolidation Inventory ( ICI )	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It describes the construction of the 35-item Identity Consolidation Inventory ( ICI ) and , as an appendix to the paper , includes the final version of this questionnaire .
	manualset3
105494	4	401698	13	NULL	NULL	0	NULL	appendix to the paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	It describes the construction of the 35-item Identity Consolidation Inventory ( ICI ) and , as an appendix to the paper , includes the final version of this questionnaire .
	manualset3
105495	5	401698	13	NULL	NULL	0	NULL	final version	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	It describes the construction of the 35-item Identity Consolidation Inventory ( ICI ) and , as an appendix to the paper , includes the final version of this questionnaire .
	manualset3
105496	6	401698	13	NULL	NULL	0	NULL	questionnaire	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	It describes the construction of the 35-item Identity Consolidation Inventory ( ICI ) and , as an appendix to the paper , includes the final version of this questionnaire .
	manualset3
105497	1	401699	13	NULL	NULL	0	NULL	 age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It did not significantly correlate with age and was more common in women .
	manualset3
105498	2	401699	13	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It did not significantly correlate with age and was more common in women .
	manualset3
105499	1	401700	13	NULL	NULL	0	NULL	stories	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It does this by exploring the stories of ` healing ' and ` survival ' produced by people who have undergone traumatic experiences such as childhood sexual abuse and a HIV positive diagnosis .
	manualset3
105500	2	401700	13	NULL	NULL	0	NULL	healing 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It does this by exploring the stories of ` healing ' and ` survival ' produced by people who have undergone traumatic experiences such as childhood sexual abuse and a HIV positive diagnosis .
	manualset3
105501	3	401700	13	NULL	NULL	0	NULL	 survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It does this by exploring the stories of ` healing ' and ` survival ' produced by people who have undergone traumatic experiences such as childhood sexual abuse and a HIV positive diagnosis .
	manualset3
105502	4	401700	13	NULL	NULL	0	NULL	people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It does this by exploring the stories of ` healing ' and ` survival ' produced by people who have undergone traumatic experiences such as childhood sexual abuse and a HIV positive diagnosis .
	manualset3
105503	5	401700	13	NULL	NULL	0	NULL	traumatic experiences	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It does this by exploring the stories of ` healing ' and ` survival ' produced by people who have undergone traumatic experiences such as childhood sexual abuse and a HIV positive diagnosis .
	manualset3
105504	6	401700	13	NULL	NULL	0	NULL	childhood sexual abuse 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It does this by exploring the stories of ` healing ' and ` survival ' produced by people who have undergone traumatic experiences such as childhood sexual abuse and a HIV positive diagnosis .
	manualset3
105505	7	401700	13	NULL	NULL	0	NULL	HIV positive diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It does this by exploring the stories of ` healing ' and ` survival ' produced by people who have undergone traumatic experiences such as childhood sexual abuse and a HIV positive diagnosis .
	manualset3
105506	1	401701	13	NULL	NULL	0	NULL	 sphingomyelinase C  	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It encodes a sphingomyelinase C ( SMase ) highly similar ( ) 50 % identity ) to the SMases from Staphylococcus aureus ( beta-toxin ) , Bacillus cereus and Leptospira interrogans .
	manualset3
105507	2	401701	13	NULL	NULL	0	NULL	SMase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It encodes a sphingomyelinase C ( SMase ) highly similar ( ) 50 % identity ) to the SMases from Staphylococcus aureus ( beta-toxin ) , Bacillus cereus and Leptospira interrogans .
	manualset3
105508	3	401701	13	NULL	NULL	0	NULL	50 % identity	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It encodes a sphingomyelinase C ( SMase ) highly similar ( ) 50 % identity ) to the SMases from Staphylococcus aureus ( beta-toxin ) , Bacillus cereus and Leptospira interrogans .
	manualset3
105509	4	401701	13	NULL	NULL	0	NULL	SMases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It encodes a sphingomyelinase C ( SMase ) highly similar ( ) 50 % identity ) to the SMases from Staphylococcus aureus ( beta-toxin ) , Bacillus cereus and Leptospira interrogans .
	manualset3
105510	5	401701	13	NULL	NULL	0	NULL	Staphylococcus aureus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It encodes a sphingomyelinase C ( SMase ) highly similar ( ) 50 % identity ) to the SMases from Staphylococcus aureus ( beta-toxin ) , Bacillus cereus and Leptospira interrogans .
	manualset3
105511	6	401701	13	NULL	NULL	0	NULL	beta-toxin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It encodes a sphingomyelinase C ( SMase ) highly similar ( ) 50 % identity ) to the SMases from Staphylococcus aureus ( beta-toxin ) , Bacillus cereus and Leptospira interrogans .
	manualset3
105512	7	401701	13	NULL	NULL	0	NULL	Bacillus cereus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It encodes a sphingomyelinase C ( SMase ) highly similar ( ) 50 % identity ) to the SMases from Staphylococcus aureus ( beta-toxin ) , Bacillus cereus and Leptospira interrogans .
	manualset3
105513	8	401701	13	NULL	NULL	0	NULL	Leptospira interrogans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It encodes a sphingomyelinase C ( SMase ) highly similar ( ) 50 % identity ) to the SMases from Staphylococcus aureus ( beta-toxin ) , Bacillus cereus and Leptospira interrogans .
	manualset3
105514	1	401702	13	NULL	NULL	0	NULL	 affinity 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	It exhibited little or no affinity for kappa opioid , PCP , and dopamine-D2 receptors .
	manualset3
105515	2	401702	13	NULL	NULL	0	NULL	kappa opioid receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It exhibited little or no affinity for kappa opioid , PCP , and dopamine-D2 receptors .
	manualset3
105516	3	401702	13	NULL	NULL	0	NULL	PCP receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It exhibited little or no affinity for kappa opioid , PCP , and dopamine-D2 receptors .
	manualset3
105517	4	401702	13	NULL	NULL	0	NULL	dopamine-D2 receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It exhibited little or no affinity for kappa opioid , PCP , and dopamine-D2 receptors .
	manualset3
105518	1	401703	13	NULL	NULL	0	NULL	5 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	5 Trandolapril ( 3 mg kg ( -1 ) day ( -1 ) ) was orally administered from the 2nd to 8th week after the operation .
	manualset3
105519	2	401703	13	NULL	NULL	0	NULL	Trandolapril	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	5 Trandolapril ( 3 mg kg ( -1 ) day ( -1 ) ) was orally administered from the 2nd to 8th week after the operation .
	manualset3
105520	3	401703	13	NULL	NULL	0	NULL	3 mg kg ( -1 ) day ( -1 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	5 Trandolapril ( 3 mg kg ( -1 ) day ( -1 ) ) was orally administered from the 2nd to 8th week after the operation .
	manualset3
105521	4	401703	13	NULL	NULL	0	NULL	2nd to 8th week	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	5 Trandolapril ( 3 mg kg ( -1 ) day ( -1 ) ) was orally administered from the 2nd to 8th week after the operation .
	manualset3
105522	5	401703	13	NULL	NULL	0	NULL	operation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	5 Trandolapril ( 3 mg kg ( -1 ) day ( -1 ) ) was orally administered from the 2nd to 8th week after the operation .
	manualset3
105523	1	401704	13	NULL	NULL	0	NULL	conceptual framework 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It follows from this conceptual framework that therapists must constantly monitor their own contributions from past relationships as well as the aspects of countertransference evoked by the patient 's behavior .
	manualset3
105524	2	401704	13	NULL	NULL	0	NULL	therapists 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It follows from this conceptual framework that therapists must constantly monitor their own contributions from past relationships as well as the aspects of countertransference evoked by the patient 's behavior .
	manualset3
105525	3	401704	13	NULL	NULL	0	NULL	monitor	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It follows from this conceptual framework that therapists must constantly monitor their own contributions from past relationships as well as the aspects of countertransference evoked by the patient 's behavior .
	manualset3
105526	4	401704	13	NULL	NULL	0	NULL	contributions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It follows from this conceptual framework that therapists must constantly monitor their own contributions from past relationships as well as the aspects of countertransference evoked by the patient 's behavior .
	manualset3
105527	5	401704	13	NULL	NULL	0	NULL	past	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	It follows from this conceptual framework that therapists must constantly monitor their own contributions from past relationships as well as the aspects of countertransference evoked by the patient 's behavior .
	manualset3
105528	6	401704	13	NULL	NULL	0	NULL	relationships 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	It follows from this conceptual framework that therapists must constantly monitor their own contributions from past relationships as well as the aspects of countertransference evoked by the patient 's behavior .
	manualset3
105529	7	401704	13	NULL	NULL	0	NULL	aspects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It follows from this conceptual framework that therapists must constantly monitor their own contributions from past relationships as well as the aspects of countertransference evoked by the patient 's behavior .
	manualset3
105530	8	401704	13	NULL	NULL	0	NULL	countertransference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It follows from this conceptual framework that therapists must constantly monitor their own contributions from past relationships as well as the aspects of countertransference evoked by the patient 's behavior .
	manualset3
105531	9	401704	13	NULL	NULL	0	NULL	patient 's	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	It follows from this conceptual framework that therapists must constantly monitor their own contributions from past relationships as well as the aspects of countertransference evoked by the patient 's behavior .
	manualset3
105532	10	401704	13	NULL	NULL	0	NULL	behavior	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It follows from this conceptual framework that therapists must constantly monitor their own contributions from past relationships as well as the aspects of countertransference evoked by the patient 's behavior .
	manualset3
105533	1	401705	13	NULL	NULL	0	NULL	small branches	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It gave off small branches to the uncus , as well as a large parahippocampal artery , the accessory anterior temporal artery , and the anterior hippocampal artery .
	manualset3
105534	2	401705	13	NULL	NULL	0	NULL	 uncus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It gave off small branches to the uncus , as well as a large parahippocampal artery , the accessory anterior temporal artery , and the anterior hippocampal artery .
	manualset3
105535	3	401705	13	NULL	NULL	0	NULL	 large parahippocampal artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It gave off small branches to the uncus , as well as a large parahippocampal artery , the accessory anterior temporal artery , and the anterior hippocampal artery .
	manualset3
105536	4	401705	13	NULL	NULL	0	NULL	accessory anterior temporal artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It gave off small branches to the uncus , as well as a large parahippocampal artery , the accessory anterior temporal artery , and the anterior hippocampal artery .
	manualset3
105537	5	401705	13	NULL	NULL	0	NULL	anterior hippocampal artery 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It gave off small branches to the uncus , as well as a large parahippocampal artery , the accessory anterior temporal artery , and the anterior hippocampal artery .
	manualset3
105538	1	401706	13	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	It has also been possible to examine the relationship between drug sensitivity and the phenotypic and genotypic properties of these clonal cell lines .
	manualset3
105539	2	401706	13	NULL	NULL	NULL	NULL	drug sensitivity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It has also been possible to examine the relationship between drug sensitivity and the phenotypic and genotypic properties of these clonal cell lines .
	manualset3
105540	3	401706	13	NULL	NULL	NULL	NULL	phenotypic properties	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It has also been possible to examine the relationship between drug sensitivity and the phenotypic and genotypic properties of these clonal cell lines .
	manualset3
105541	4	401706	13	NULL	NULL	NULL	NULL	genotypic properties	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It has also been possible to examine the relationship between drug sensitivity and the phenotypic and genotypic properties of these clonal cell lines .
	manualset3
105542	5	401706	13	NULL	NULL	0	NULL	clonal cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It has also been possible to examine the relationship between drug sensitivity and the phenotypic and genotypic properties of these clonal cell lines .
	manualset3
105543	1	401707	13	NULL	NULL	0	NULL	 transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It has also been shown to activate transcription from rRNA promoters both in vitro and in vivo .
	manualset3
105544	2	401707	13	NULL	NULL	0	NULL	rRNA promoters 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It has also been shown to activate transcription from rRNA promoters both in vitro and in vivo .
	manualset3
105545	1	401708	13	NULL	NULL	0	NULL	essential amino acid ( EAA ) solution	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been claimed that conventional essential amino acid ( EAA ) solution may give rise to adverse effects such as hyperammonemia , in acute renal failure ( ARF ) .
	manualset3
105546	2	401708	13	NULL	NULL	0	NULL	rise 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been claimed that conventional essential amino acid ( EAA ) solution may give rise to adverse effects such as hyperammonemia , in acute renal failure ( ARF ) .
	manualset3
105547	3	401708	13	NULL	NULL	0	NULL	adverse effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been claimed that conventional essential amino acid ( EAA ) solution may give rise to adverse effects such as hyperammonemia , in acute renal failure ( ARF ) .
	manualset3
105548	4	401708	13	NULL	NULL	0	NULL	 hyperammonemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been claimed that conventional essential amino acid ( EAA ) solution may give rise to adverse effects such as hyperammonemia , in acute renal failure ( ARF ) .
	manualset3
105549	5	401708	13	NULL	NULL	0	NULL	acute renal failure ( ARF )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been claimed that conventional essential amino acid ( EAA ) solution may give rise to adverse effects such as hyperammonemia , in acute renal failure ( ARF ) .
	manualset3
105550	1	401709	13	NULL	NULL	0	NULL	polymorphisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been consistently demonstrated that polymorphisms in the genes that encode for apolipoproteins A5 , C3 and E , for the cholesterol ester transporter proteins ( CETP ) , and in the ATP binding cassette type A1 ( ABCA1 ) influence the development of dyslipidemia in patients treated with antiretroviral drugs , particularly if the therapeutic regimen includes protease inhibitors .
	manualset3
105551	2	401709	13	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been consistently demonstrated that polymorphisms in the genes that encode for apolipoproteins A5 , C3 and E , for the cholesterol ester transporter proteins ( CETP ) , and in the ATP binding cassette type A1 ( ABCA1 ) influence the development of dyslipidemia in patients treated with antiretroviral drugs , particularly if the therapeutic regimen includes protease inhibitors .
	manualset3
105552	3	401709	13	NULL	NULL	0	NULL	 apolipoproteins A5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been consistently demonstrated that polymorphisms in the genes that encode for apolipoproteins A5 , C3 and E , for the cholesterol ester transporter proteins ( CETP ) , and in the ATP binding cassette type A1 ( ABCA1 ) influence the development of dyslipidemia in patients treated with antiretroviral drugs , particularly if the therapeutic regimen includes protease inhibitors .
	manualset3
105553	4	401709	13	NULL	NULL	0	NULL	apolipoproteins C3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been consistently demonstrated that polymorphisms in the genes that encode for apolipoproteins A5 , C3 and E , for the cholesterol ester transporter proteins ( CETP ) , and in the ATP binding cassette type A1 ( ABCA1 ) influence the development of dyslipidemia in patients treated with antiretroviral drugs , particularly if the therapeutic regimen includes protease inhibitors .
	manualset3
105554	5	401709	13	NULL	NULL	0	NULL	apolipoproteins E	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been consistently demonstrated that polymorphisms in the genes that encode for apolipoproteins A5 , C3 and E , for the cholesterol ester transporter proteins ( CETP ) , and in the ATP binding cassette type A1 ( ABCA1 ) influence the development of dyslipidemia in patients treated with antiretroviral drugs , particularly if the therapeutic regimen includes protease inhibitors .
	manualset3
105555	6	401709	13	NULL	NULL	0	NULL	cholesterol ester transporter proteins ( CETP ) 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been consistently demonstrated that polymorphisms in the genes that encode for apolipoproteins A5 , C3 and E , for the cholesterol ester transporter proteins ( CETP ) , and in the ATP binding cassette type A1 ( ABCA1 ) influence the development of dyslipidemia in patients treated with antiretroviral drugs , particularly if the therapeutic regimen includes protease inhibitors .
	manualset3
105556	7	401709	13	NULL	NULL	0	NULL	ATP binding cassette type A1 ( ABCA1 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been consistently demonstrated that polymorphisms in the genes that encode for apolipoproteins A5 , C3 and E , for the cholesterol ester transporter proteins ( CETP ) , and in the ATP binding cassette type A1 ( ABCA1 ) influence the development of dyslipidemia in patients treated with antiretroviral drugs , particularly if the therapeutic regimen includes protease inhibitors .
	manualset3
105558	9	401709	13	NULL	NULL	0	NULL	development	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been consistently demonstrated that polymorphisms in the genes that encode for apolipoproteins A5 , C3 and E , for the cholesterol ester transporter proteins ( CETP ) , and in the ATP binding cassette type A1 ( ABCA1 ) influence the development of dyslipidemia in patients treated with antiretroviral drugs , particularly if the therapeutic regimen includes protease inhibitors .
	manualset3
105559	10	401709	13	NULL	NULL	0	NULL	dyslipidemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been consistently demonstrated that polymorphisms in the genes that encode for apolipoproteins A5 , C3 and E , for the cholesterol ester transporter proteins ( CETP ) , and in the ATP binding cassette type A1 ( ABCA1 ) influence the development of dyslipidemia in patients treated with antiretroviral drugs , particularly if the therapeutic regimen includes protease inhibitors .
	manualset3
105560	11	401709	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been consistently demonstrated that polymorphisms in the genes that encode for apolipoproteins A5 , C3 and E , for the cholesterol ester transporter proteins ( CETP ) , and in the ATP binding cassette type A1 ( ABCA1 ) influence the development of dyslipidemia in patients treated with antiretroviral drugs , particularly if the therapeutic regimen includes protease inhibitors .
	manualset3
105561	12	401709	13	NULL	NULL	0	NULL	antiretroviral drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been consistently demonstrated that polymorphisms in the genes that encode for apolipoproteins A5 , C3 and E , for the cholesterol ester transporter proteins ( CETP ) , and in the ATP binding cassette type A1 ( ABCA1 ) influence the development of dyslipidemia in patients treated with antiretroviral drugs , particularly if the therapeutic regimen includes protease inhibitors .
	manualset3
105562	13	401709	13	NULL	NULL	0	NULL	therapeutic regimen	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been consistently demonstrated that polymorphisms in the genes that encode for apolipoproteins A5 , C3 and E , for the cholesterol ester transporter proteins ( CETP ) , and in the ATP binding cassette type A1 ( ABCA1 ) influence the development of dyslipidemia in patients treated with antiretroviral drugs , particularly if the therapeutic regimen includes protease inhibitors .
	manualset3
105563	14	401709	13	NULL	NULL	0	NULL	 protease inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been consistently demonstrated that polymorphisms in the genes that encode for apolipoproteins A5 , C3 and E , for the cholesterol ester transporter proteins ( CETP ) , and in the ATP binding cassette type A1 ( ABCA1 ) influence the development of dyslipidemia in patients treated with antiretroviral drugs , particularly if the therapeutic regimen includes protease inhibitors .
	manualset3
105564	1	401710	13	NULL	NULL	0	NULL	Western blotting	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been determined by Western blotting to share epitopes with the gp41 viral transmembrane component of HIV-1 .
	manualset3
105565	2	401710	13	NULL	NULL	0	NULL	epitopes 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been determined by Western blotting to share epitopes with the gp41 viral transmembrane component of HIV-1 .
	manualset3
105566	3	401710	13	NULL	NULL	0	NULL	gp41	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been determined by Western blotting to share epitopes with the gp41 viral transmembrane component of HIV-1 .
	manualset3
105567	4	401710	13	NULL	NULL	0	NULL	viral transmembrane component	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been determined by Western blotting to share epitopes with the gp41 viral transmembrane component of HIV-1 .
	manualset3
105568	5	401710	13	NULL	NULL	0	NULL	HIV-1	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been determined by Western blotting to share epitopes with the gp41 viral transmembrane component of HIV-1 .
	manualset3
105569	1	401711	13	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been discovered that genes could be silenced by introducing double-stranded RNAs ( dsRNAs ) complementary to the messenger RNA sequences .
	manualset3
105570	2	401711	13	NULL	NULL	0	NULL	double-stranded RNAs ( dsRNAs )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been discovered that genes could be silenced by introducing double-stranded RNAs ( dsRNAs ) complementary to the messenger RNA sequences .
	manualset3
105571	3	401711	13	NULL	NULL	0	NULL	messenger RNA sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been discovered that genes could be silenced by introducing double-stranded RNAs ( dsRNAs ) complementary to the messenger RNA sequences .
	manualset3
105572	1	401712	13	NULL	NULL	0	NULL	( R ) - ( alpha - ( 2 ) H ( 1 ) ) - alcohols	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been found that with ( R ) - ( alpha - ( 2 ) H ( 1 ) ) - alcohols , the oxidation involves almost exclusively the cleavage of the C-H bond , whereas in the case of the oxidation of ( S ) - ( alpha - ( 2 ) H ( 1 ) ) - alcohols , the C-D bond is preferentially broken .
	manualset3
105573	2	401712	13	NULL	NULL	0	NULL	oxidation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been found that with ( R ) - ( alpha - ( 2 ) H ( 1 ) ) - alcohols , the oxidation involves almost exclusively the cleavage of the C-H bond , whereas in the case of the oxidation of ( S ) - ( alpha - ( 2 ) H ( 1 ) ) - alcohols , the C-D bond is preferentially broken .
	manualset3
105574	3	401712	13	NULL	NULL	0	NULL	cleavage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been found that with ( R ) - ( alpha - ( 2 ) H ( 1 ) ) - alcohols , the oxidation involves almost exclusively the cleavage of the C-H bond , whereas in the case of the oxidation of ( S ) - ( alpha - ( 2 ) H ( 1 ) ) - alcohols , the C-D bond is preferentially broken .
	manualset3
105575	4	401712	13	NULL	NULL	0	NULL	 C-H bond	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been found that with ( R ) - ( alpha - ( 2 ) H ( 1 ) ) - alcohols , the oxidation involves almost exclusively the cleavage of the C-H bond , whereas in the case of the oxidation of ( S ) - ( alpha - ( 2 ) H ( 1 ) ) - alcohols , the C-D bond is preferentially broken .
	manualset3
105576	5	401712	13	NULL	NULL	0	NULL	oxidation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been found that with ( R ) - ( alpha - ( 2 ) H ( 1 ) ) - alcohols , the oxidation involves almost exclusively the cleavage of the C-H bond , whereas in the case of the oxidation of ( S ) - ( alpha - ( 2 ) H ( 1 ) ) - alcohols , the C-D bond is preferentially broken .
	manualset3
105577	6	401712	13	NULL	NULL	0	NULL	( S ) - ( alpha - ( 2 ) H ( 1 ) ) - alcohols	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been found that with ( R ) - ( alpha - ( 2 ) H ( 1 ) ) - alcohols , the oxidation involves almost exclusively the cleavage of the C-H bond , whereas in the case of the oxidation of ( S ) - ( alpha - ( 2 ) H ( 1 ) ) - alcohols , the C-D bond is preferentially broken .
	manualset3
105578	7	401712	13	NULL	NULL	0	NULL	 C-D bond	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been found that with ( R ) - ( alpha - ( 2 ) H ( 1 ) ) - alcohols , the oxidation involves almost exclusively the cleavage of the C-H bond , whereas in the case of the oxidation of ( S ) - ( alpha - ( 2 ) H ( 1 ) ) - alcohols , the C-D bond is preferentially broken .
	manualset3
105579	1	401713	13	NULL	NULL	0	NULL	calcium influx	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been hypothesized that calcium influx into axons plays a major role in the pathophysiology of DAI .
	manualset3
105580	2	401713	13	NULL	NULL	0	NULL	axons	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been hypothesized that calcium influx into axons plays a major role in the pathophysiology of DAI .
	manualset3
105581	3	401713	13	NULL	NULL	0	NULL	major role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been hypothesized that calcium influx into axons plays a major role in the pathophysiology of DAI .
	manualset3
105582	4	401713	13	NULL	NULL	0	NULL	pathophysiology of DAI	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been hypothesized that calcium influx into axons plays a major role in the pathophysiology of DAI .
	manualset3
105583	1	401714	13	NULL	NULL	NULL	NULL	 increases	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It has been hypothesized that these increases are due to the reduction of lysine-poor zeins and a pleiotropic increase in the lysine-rich non-zein proteins .
	manualset3
105584	2	401714	13	NULL	NULL	0	NULL	reduction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been hypothesized that these increases are due to the reduction of lysine-poor zeins and a pleiotropic increase in the lysine-rich non-zein proteins .
	manualset3
105585	3	401714	13	NULL	NULL	0	NULL	lysine-poor zeins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been hypothesized that these increases are due to the reduction of lysine-poor zeins and a pleiotropic increase in the lysine-rich non-zein proteins .
	manualset3
105586	4	401714	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been hypothesized that these increases are due to the reduction of lysine-poor zeins and a pleiotropic increase in the lysine-rich non-zein proteins .
	manualset3
105587	5	401714	13	NULL	NULL	0	NULL	lysine-rich non-zein proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been hypothesized that these increases are due to the reduction of lysine-poor zeins and a pleiotropic increase in the lysine-rich non-zein proteins .
	manualset3
105588	1	401715	13	NULL	NULL	0	NULL	30 years	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been more than 30 years since the introduction of endoscopic sphincterotomy for the management of choledocholithiasis .
	manualset3
105589	2	401715	13	NULL	NULL	0	NULL	introduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been more than 30 years since the introduction of endoscopic sphincterotomy for the management of choledocholithiasis .
	manualset3
105590	3	401715	13	NULL	NULL	0	NULL	endoscopic sphincterotomy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been more than 30 years since the introduction of endoscopic sphincterotomy for the management of choledocholithiasis .
	manualset3
105591	4	401715	13	NULL	NULL	0	NULL	management 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been more than 30 years since the introduction of endoscopic sphincterotomy for the management of choledocholithiasis .
	manualset3
105592	5	401715	13	NULL	NULL	0	NULL	choledocholithiasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been more than 30 years since the introduction of endoscopic sphincterotomy for the management of choledocholithiasis .
	manualset3
105593	1	401716	13	NULL	NULL	0	NULL	alleles	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been observed that certain rare alleles of the c-Ha-ras gene occur more frequently in patients with certain malignant tumors than in healthy individuals , suggesting that these alleles may serve as markers for particular types of cancer .
	manualset3
105594	2	401716	13	NULL	NULL	0	NULL	c-Ha-ras gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been observed that certain rare alleles of the c-Ha-ras gene occur more frequently in patients with certain malignant tumors than in healthy individuals , suggesting that these alleles may serve as markers for particular types of cancer .
	manualset3
105595	3	401716	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been observed that certain rare alleles of the c-Ha-ras gene occur more frequently in patients with certain malignant tumors than in healthy individuals , suggesting that these alleles may serve as markers for particular types of cancer .
	manualset3
105596	4	401716	13	NULL	NULL	0	NULL	malignant tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been observed that certain rare alleles of the c-Ha-ras gene occur more frequently in patients with certain malignant tumors than in healthy individuals , suggesting that these alleles may serve as markers for particular types of cancer .
	manualset3
105597	5	401716	13	NULL	NULL	0	NULL	healthy individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been observed that certain rare alleles of the c-Ha-ras gene occur more frequently in patients with certain malignant tumors than in healthy individuals , suggesting that these alleles may serve as markers for particular types of cancer .
	manualset3
105598	6	401716	13	NULL	NULL	0	NULL	alleles 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been observed that certain rare alleles of the c-Ha-ras gene occur more frequently in patients with certain malignant tumors than in healthy individuals , suggesting that these alleles may serve as markers for particular types of cancer .
	manualset3
105599	7	401716	13	NULL	NULL	NULL	NULL	markers	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It has been observed that certain rare alleles of the c-Ha-ras gene occur more frequently in patients with certain malignant tumors than in healthy individuals , suggesting that these alleles may serve as markers for particular types of cancer .
	manualset3
105600	8	401716	13	NULL	NULL	0	NULL	particular types of cancer	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been observed that certain rare alleles of the c-Ha-ras gene occur more frequently in patients with certain malignant tumors than in healthy individuals , suggesting that these alleles may serve as markers for particular types of cancer .
	manualset3
105601	1	401717	13	NULL	NULL	0	NULL	HIV-infected patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been postulated that HIV-infected patients may have special types of intestinal infections , and that immune activation from such parasites may affect the progression of HIV disease .
	manualset3
105602	2	401717	13	NULL	NULL	0	NULL	special types of intestinal infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been postulated that HIV-infected patients may have special types of intestinal infections , and that immune activation from such parasites may affect the progression of HIV disease .
	manualset3
105603	3	401717	13	NULL	NULL	0	NULL	immune activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been postulated that HIV-infected patients may have special types of intestinal infections , and that immune activation from such parasites may affect the progression of HIV disease .
	manualset3
105604	4	401717	13	NULL	NULL	0	NULL	parasites 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been postulated that HIV-infected patients may have special types of intestinal infections , and that immune activation from such parasites may affect the progression of HIV disease .
	manualset3
105605	5	401717	13	NULL	NULL	0	NULL	progression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been postulated that HIV-infected patients may have special types of intestinal infections , and that immune activation from such parasites may affect the progression of HIV disease .
	manualset3
105606	6	401717	13	NULL	NULL	0	NULL	HIV disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been postulated that HIV-infected patients may have special types of intestinal infections , and that immune activation from such parasites may affect the progression of HIV disease .
	manualset3
105607	1	401718	13	NULL	NULL	0	NULL	domain movement 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been proposed that domain movement , resulting in closure of the active site cleft , is essential for the catalytic function of PGK .
	manualset3
105608	2	401718	13	NULL	NULL	0	NULL	closure	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been proposed that domain movement , resulting in closure of the active site cleft , is essential for the catalytic function of PGK .
	manualset3
105609	3	401718	13	NULL	NULL	0	NULL	active site cleft	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been proposed that domain movement , resulting in closure of the active site cleft , is essential for the catalytic function of PGK .
	manualset3
105610	4	401718	13	NULL	NULL	0	NULL	catalytic function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been proposed that domain movement , resulting in closure of the active site cleft , is essential for the catalytic function of PGK .
	manualset3
105611	5	401718	13	NULL	NULL	0	NULL	PGK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been proposed that domain movement , resulting in closure of the active site cleft , is essential for the catalytic function of PGK .
	manualset3
105612	1	401719	13	NULL	NULL	0	NULL	somatosensory stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been proposed that somatosensory stimulation in the form of electromyographically triggered neuromuscular electrical stimulation ( NMES ) to the peripheral nerve can influence functional measures of motor performance in subjects with stroke and can additionally produce changes in cortical excitability .
	manualset3
105613	2	401719	13	NULL	NULL	0	NULL	neuromuscular electrical stimulation ( NMES )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been proposed that somatosensory stimulation in the form of electromyographically triggered neuromuscular electrical stimulation ( NMES ) to the peripheral nerve can influence functional measures of motor performance in subjects with stroke and can additionally produce changes in cortical excitability .
	manualset3
105614	3	401719	13	NULL	NULL	0	NULL	peripheral nerve	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been proposed that somatosensory stimulation in the form of electromyographically triggered neuromuscular electrical stimulation ( NMES ) to the peripheral nerve can influence functional measures of motor performance in subjects with stroke and can additionally produce changes in cortical excitability .
	manualset3
105615	4	401719	13	NULL	NULL	0	NULL	functional measures	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been proposed that somatosensory stimulation in the form of electromyographically triggered neuromuscular electrical stimulation ( NMES ) to the peripheral nerve can influence functional measures of motor performance in subjects with stroke and can additionally produce changes in cortical excitability .
	manualset3
105616	5	401719	13	NULL	NULL	0	NULL	motor performance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been proposed that somatosensory stimulation in the form of electromyographically triggered neuromuscular electrical stimulation ( NMES ) to the peripheral nerve can influence functional measures of motor performance in subjects with stroke and can additionally produce changes in cortical excitability .
	manualset3
105617	6	401719	13	NULL	NULL	0	NULL	subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been proposed that somatosensory stimulation in the form of electromyographically triggered neuromuscular electrical stimulation ( NMES ) to the peripheral nerve can influence functional measures of motor performance in subjects with stroke and can additionally produce changes in cortical excitability .
	manualset3
105618	7	401719	13	NULL	NULL	0	NULL	stroke	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been proposed that somatosensory stimulation in the form of electromyographically triggered neuromuscular electrical stimulation ( NMES ) to the peripheral nerve can influence functional measures of motor performance in subjects with stroke and can additionally produce changes in cortical excitability .
	manualset3
105619	8	401719	13	NULL	NULL	0	NULL	changes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been proposed that somatosensory stimulation in the form of electromyographically triggered neuromuscular electrical stimulation ( NMES ) to the peripheral nerve can influence functional measures of motor performance in subjects with stroke and can additionally produce changes in cortical excitability .
	manualset3
105620	9	401719	13	NULL	NULL	0	NULL	cortical excitability 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been proposed that somatosensory stimulation in the form of electromyographically triggered neuromuscular electrical stimulation ( NMES ) to the peripheral nerve can influence functional measures of motor performance in subjects with stroke and can additionally produce changes in cortical excitability .
	manualset3
105621	1	401720	13	NULL	NULL	0	NULL	51 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	51 % , 22.4 % and 46.9 % of those were colonized at IV , ETV and FUV , respectively ( p = 0.007 ) .
	manualset3
105622	2	401720	13	NULL	NULL	0	NULL	22.4 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	51 % , 22.4 % and 46.9 % of those were colonized at IV , ETV and FUV , respectively ( p = 0.007 ) .
	manualset3
105623	3	401720	13	NULL	NULL	0	NULL	46.9 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	51 % , 22.4 % and 46.9 % of those were colonized at IV , ETV and FUV , respectively ( p = 0.007 ) .
	manualset3
105624	4	401720	13	NULL	NULL	0	NULL	IV	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	51 % , 22.4 % and 46.9 % of those were colonized at IV , ETV and FUV , respectively ( p = 0.007 ) .
	manualset3
105625	5	401720	13	NULL	NULL	0	NULL	ETV	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	51 % , 22.4 % and 46.9 % of those were colonized at IV , ETV and FUV , respectively ( p = 0.007 ) .
	manualset3
105626	6	401720	13	NULL	NULL	0	NULL	FUV	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	51 % , 22.4 % and 46.9 % of those were colonized at IV , ETV and FUV , respectively ( p = 0.007 ) .
	manualset3
105627	7	401720	13	NULL	NULL	0	NULL	p = 0.007	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	51 % , 22.4 % and 46.9 % of those were colonized at IV , ETV and FUV , respectively ( p = 0.007 ) .
	manualset3
105628	1	401721	13	NULL	NULL	0	NULL	hospitals	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been recently investigated at many hospitals and institutes , mainly in Europe and the USA .
	manualset3
105629	2	401721	13	NULL	NULL	0	NULL	institutes	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been recently investigated at many hospitals and institutes , mainly in Europe and the USA .
	manualset3
105630	3	401721	13	NULL	NULL	0	NULL	Europe	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been recently investigated at many hospitals and institutes , mainly in Europe and the USA .
	manualset3
105631	4	401721	13	NULL	NULL	0	NULL	 USA	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been recently investigated at many hospitals and institutes , mainly in Europe and the USA .
	manualset3
105632	1	401722	13	NULL	NULL	0	NULL	second extracellular loop	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been recently proposed that the second extracellular loop of the human bradykinin ( BK ) B1 receptor ( B1R ) contains a conserved HExxH motif also present in peptidases possessing a Zn2 + prosthetic group , such as angiotensin converting enzyme ( ACE ) , and that ACE inhibitors directly activate B1R signaling in endothelial cells .
	manualset3
105633	2	401722	13	NULL	NULL	0	NULL	 human bradykinin ( BK ) B1 receptor ( B1R ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been recently proposed that the second extracellular loop of the human bradykinin ( BK ) B1 receptor ( B1R ) contains a conserved HExxH motif also present in peptidases possessing a Zn2 + prosthetic group , such as angiotensin converting enzyme ( ACE ) , and that ACE inhibitors directly activate B1R signaling in endothelial cells .
	manualset3
105634	3	401722	13	NULL	NULL	0	NULL	 HExxH motif	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been recently proposed that the second extracellular loop of the human bradykinin ( BK ) B1 receptor ( B1R ) contains a conserved HExxH motif also present in peptidases possessing a Zn2 + prosthetic group , such as angiotensin converting enzyme ( ACE ) , and that ACE inhibitors directly activate B1R signaling in endothelial cells .
	manualset3
105635	4	401722	13	NULL	NULL	0	NULL	peptidases 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been recently proposed that the second extracellular loop of the human bradykinin ( BK ) B1 receptor ( B1R ) contains a conserved HExxH motif also present in peptidases possessing a Zn2 + prosthetic group , such as angiotensin converting enzyme ( ACE ) , and that ACE inhibitors directly activate B1R signaling in endothelial cells .
	manualset3
105636	5	401722	13	NULL	NULL	0	NULL	Zn2 + prosthetic group 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been recently proposed that the second extracellular loop of the human bradykinin ( BK ) B1 receptor ( B1R ) contains a conserved HExxH motif also present in peptidases possessing a Zn2 + prosthetic group , such as angiotensin converting enzyme ( ACE ) , and that ACE inhibitors directly activate B1R signaling in endothelial cells .
	manualset3
105637	6	401722	13	NULL	NULL	0	NULL	angiotensin converting enzyme ( ACE ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been recently proposed that the second extracellular loop of the human bradykinin ( BK ) B1 receptor ( B1R ) contains a conserved HExxH motif also present in peptidases possessing a Zn2 + prosthetic group , such as angiotensin converting enzyme ( ACE ) , and that ACE inhibitors directly activate B1R signaling in endothelial cells .
	manualset3
105638	7	401722	13	NULL	NULL	0	NULL	ACE inhibitors 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been recently proposed that the second extracellular loop of the human bradykinin ( BK ) B1 receptor ( B1R ) contains a conserved HExxH motif also present in peptidases possessing a Zn2 + prosthetic group , such as angiotensin converting enzyme ( ACE ) , and that ACE inhibitors directly activate B1R signaling in endothelial cells .
	manualset3
105639	8	401722	13	NULL	NULL	0	NULL	B1R signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been recently proposed that the second extracellular loop of the human bradykinin ( BK ) B1 receptor ( B1R ) contains a conserved HExxH motif also present in peptidases possessing a Zn2 + prosthetic group , such as angiotensin converting enzyme ( ACE ) , and that ACE inhibitors directly activate B1R signaling in endothelial cells .
	manualset3
105640	9	401722	13	NULL	NULL	0	NULL	endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been recently proposed that the second extracellular loop of the human bradykinin ( BK ) B1 receptor ( B1R ) contains a conserved HExxH motif also present in peptidases possessing a Zn2 + prosthetic group , such as angiotensin converting enzyme ( ACE ) , and that ACE inhibitors directly activate B1R signaling in endothelial cells .
	manualset3
105641	1	401723	13	NULL	NULL	0	NULL	anaerobic threshold ( AT )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been recognized that anaerobic threshold ( AT ) and maximal oxygen uptake ( VO2 max ) may be useful in identifying one 's exercise tolerance .
	manualset3
105642	2	401723	13	NULL	NULL	0	NULL	maximal oxygen uptake ( VO2 max )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been recognized that anaerobic threshold ( AT ) and maximal oxygen uptake ( VO2 max ) may be useful in identifying one 's exercise tolerance .
	manualset3
105643	3	401723	13	NULL	NULL	0	NULL	exercise tolerance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been recognized that anaerobic threshold ( AT ) and maximal oxygen uptake ( VO2 max ) may be useful in identifying one 's exercise tolerance .
	manualset3
105644	1	401724	13	NULL	NULL	0	NULL	ETs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been reported that ETs play a pivotal role in the pathogenesis of asthma , chronic obstructive pulmonary disease , bronchiolitis obliterans and other important airway diseases .
	manualset3
105645	2	401724	13	NULL	NULL	0	NULL	pivotal role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been reported that ETs play a pivotal role in the pathogenesis of asthma , chronic obstructive pulmonary disease , bronchiolitis obliterans and other important airway diseases .
	manualset3
105646	3	401724	13	NULL	NULL	0	NULL	pathogenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been reported that ETs play a pivotal role in the pathogenesis of asthma , chronic obstructive pulmonary disease , bronchiolitis obliterans and other important airway diseases .
	manualset3
105647	4	401724	13	NULL	NULL	NULL	NULL	asthma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It has been reported that ETs play a pivotal role in the pathogenesis of asthma , chronic obstructive pulmonary disease , bronchiolitis obliterans and other important airway diseases .
	manualset3
105648	5	401724	13	NULL	NULL	0	NULL	chronic obstructive pulmonary disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been reported that ETs play a pivotal role in the pathogenesis of asthma , chronic obstructive pulmonary disease , bronchiolitis obliterans and other important airway diseases .
	manualset3
105649	6	401724	13	NULL	NULL	0	NULL	bronchiolitis obliterans 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been reported that ETs play a pivotal role in the pathogenesis of asthma , chronic obstructive pulmonary disease , bronchiolitis obliterans and other important airway diseases .
	manualset3
105650	7	401724	13	NULL	NULL	0	NULL	airway diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been reported that ETs play a pivotal role in the pathogenesis of asthma , chronic obstructive pulmonary disease , bronchiolitis obliterans and other important airway diseases .
	manualset3
105651	1	401725	13	NULL	NULL	0	NULL	plant virus-derived small interfering RNAs ( vsiRNAs ) 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been reported that plant virus-derived small interfering RNAs ( vsiRNAs ) originated predominantly from structured single-stranded viral RNA of a positive single-stranded RNA virus replicating in the cytoplasm and from the nuclear stem-loop 35S leader RNA of a double-stranded DNA ( dsDNA ) virus .
	manualset3
105652	2	401725	13	NULL	NULL	0	NULL	 single-stranded viral RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been reported that plant virus-derived small interfering RNAs ( vsiRNAs ) originated predominantly from structured single-stranded viral RNA of a positive single-stranded RNA virus replicating in the cytoplasm and from the nuclear stem-loop 35S leader RNA of a double-stranded DNA ( dsDNA ) virus .
	manualset3
105653	3	401725	13	NULL	NULL	0	NULL	positive single-stranded RNA virus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been reported that plant virus-derived small interfering RNAs ( vsiRNAs ) originated predominantly from structured single-stranded viral RNA of a positive single-stranded RNA virus replicating in the cytoplasm and from the nuclear stem-loop 35S leader RNA of a double-stranded DNA ( dsDNA ) virus .
	manualset3
105654	4	401725	13	NULL	NULL	0	NULL	cytoplasm	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been reported that plant virus-derived small interfering RNAs ( vsiRNAs ) originated predominantly from structured single-stranded viral RNA of a positive single-stranded RNA virus replicating in the cytoplasm and from the nuclear stem-loop 35S leader RNA of a double-stranded DNA ( dsDNA ) virus .
	manualset3
105655	5	401725	13	NULL	NULL	0	NULL	nuclear stem-loop 35S leader RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been reported that plant virus-derived small interfering RNAs ( vsiRNAs ) originated predominantly from structured single-stranded viral RNA of a positive single-stranded RNA virus replicating in the cytoplasm and from the nuclear stem-loop 35S leader RNA of a double-stranded DNA ( dsDNA ) virus .
	manualset3
105656	6	401725	13	NULL	NULL	0	NULL	double-stranded DNA ( dsDNA ) virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been reported that plant virus-derived small interfering RNAs ( vsiRNAs ) originated predominantly from structured single-stranded viral RNA of a positive single-stranded RNA virus replicating in the cytoplasm and from the nuclear stem-loop 35S leader RNA of a double-stranded DNA ( dsDNA ) virus .
	manualset3
105657	1	401726	13	NULL	NULL	0	NULL	irreversible alkylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been reported that the irreversible alkylation of protein cysteinyl residues is responsible for STL inhibition of several different enzymes , and second-order rate constants for the reaction of helenalin and alantolactone with glutathione were 25.1 and 1.80 mM-1 .
	manualset3
105658	2	401726	13	NULL	NULL	0	NULL	protein cysteinyl residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been reported that the irreversible alkylation of protein cysteinyl residues is responsible for STL inhibition of several different enzymes , and second-order rate constants for the reaction of helenalin and alantolactone with glutathione were 25.1 and 1.80 mM-1 .
	manualset3
105659	3	401726	13	NULL	NULL	0	NULL	STL inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been reported that the irreversible alkylation of protein cysteinyl residues is responsible for STL inhibition of several different enzymes , and second-order rate constants for the reaction of helenalin and alantolactone with glutathione were 25.1 and 1.80 mM-1 .
	manualset3
105660	4	401726	13	NULL	NULL	0	NULL	enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been reported that the irreversible alkylation of protein cysteinyl residues is responsible for STL inhibition of several different enzymes , and second-order rate constants for the reaction of helenalin and alantolactone with glutathione were 25.1 and 1.80 mM-1 .
	manualset3
105661	5	401726	13	NULL	NULL	0	NULL	second-order rate constants 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been reported that the irreversible alkylation of protein cysteinyl residues is responsible for STL inhibition of several different enzymes , and second-order rate constants for the reaction of helenalin and alantolactone with glutathione were 25.1 and 1.80 mM-1 .
	manualset3
105662	6	401726	13	NULL	NULL	0	NULL	reaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been reported that the irreversible alkylation of protein cysteinyl residues is responsible for STL inhibition of several different enzymes , and second-order rate constants for the reaction of helenalin and alantolactone with glutathione were 25.1 and 1.80 mM-1 .
	manualset3
105663	7	401726	13	NULL	NULL	NULL	NULL	helenalin	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It has been reported that the irreversible alkylation of protein cysteinyl residues is responsible for STL inhibition of several different enzymes , and second-order rate constants for the reaction of helenalin and alantolactone with glutathione were 25.1 and 1.80 mM-1 .
	manualset3
105664	8	401726	13	NULL	NULL	0	NULL	alantolactone 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been reported that the irreversible alkylation of protein cysteinyl residues is responsible for STL inhibition of several different enzymes , and second-order rate constants for the reaction of helenalin and alantolactone with glutathione were 25.1 and 1.80 mM-1 .
	manualset3
105665	9	401726	13	NULL	NULL	0	NULL	glutathione 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been reported that the irreversible alkylation of protein cysteinyl residues is responsible for STL inhibition of several different enzymes , and second-order rate constants for the reaction of helenalin and alantolactone with glutathione were 25.1 and 1.80 mM-1 .
	manualset3
105666	10	401726	13	NULL	NULL	0	NULL	25.1 mM-1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been reported that the irreversible alkylation of protein cysteinyl residues is responsible for STL inhibition of several different enzymes , and second-order rate constants for the reaction of helenalin and alantolactone with glutathione were 25.1 and 1.80 mM-1 .
	manualset3
105667	11	401726	13	NULL	NULL	0	NULL	1.80 mM-1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been reported that the irreversible alkylation of protein cysteinyl residues is responsible for STL inhibition of several different enzymes , and second-order rate constants for the reaction of helenalin and alantolactone with glutathione were 25.1 and 1.80 mM-1 .
	manualset3
105668	1	401727	13	NULL	NULL	0	NULL	essence of medicine 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been said that the essence of medicine is the reduction of uncertainty for patients and physicians ( Ludo Baghius ) .
	manualset3
105669	2	401727	13	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been said that the essence of medicine is the reduction of uncertainty for patients and physicians ( Ludo Baghius ) .
	manualset3
105670	3	401727	13	NULL	NULL	0	NULL	 uncertainty	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been said that the essence of medicine is the reduction of uncertainty for patients and physicians ( Ludo Baghius ) .
	manualset3
105671	4	401727	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been said that the essence of medicine is the reduction of uncertainty for patients and physicians ( Ludo Baghius ) .
	manualset3
105672	5	401727	13	NULL	NULL	0	NULL	physicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been said that the essence of medicine is the reduction of uncertainty for patients and physicians ( Ludo Baghius ) .
	manualset3
105673	6	401727	13	NULL	NULL	0	NULL	Ludo Baghius	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been said that the essence of medicine is the reduction of uncertainty for patients and physicians ( Ludo Baghius ) .
	manualset3
105674	1	401728	13	NULL	NULL	0	NULL	injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been shown that injection of herpes simplex virus ( HSV ) type I into the vitreous body of the eye in 18-day-old albino rabbits consistently induced encephalitis .
	manualset3
105675	2	401728	13	NULL	NULL	0	NULL	herpes simplex virus ( HSV ) type I	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been shown that injection of herpes simplex virus ( HSV ) type I into the vitreous body of the eye in 18-day-old albino rabbits consistently induced encephalitis .
	manualset3
105676	3	401728	13	NULL	NULL	0	NULL	vitreous body of the eye	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been shown that injection of herpes simplex virus ( HSV ) type I into the vitreous body of the eye in 18-day-old albino rabbits consistently induced encephalitis .
	manualset3
105677	4	401728	13	NULL	NULL	0	NULL	8-day-old albino rabbits	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been shown that injection of herpes simplex virus ( HSV ) type I into the vitreous body of the eye in 18-day-old albino rabbits consistently induced encephalitis .
	manualset3
105678	5	401728	13	NULL	NULL	0	NULL	encephalitis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been shown that injection of herpes simplex virus ( HSV ) type I into the vitreous body of the eye in 18-day-old albino rabbits consistently induced encephalitis .
	manualset3
105679	1	401729	13	NULL	NULL	0	NULL	viruses 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been shown that viruses can induce alterations in the content and distribution of cytoskeleton structures , particularly actin microfilaments and microtubules .
	manualset3
105680	2	401729	13	NULL	NULL	0	NULL	alterations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been shown that viruses can induce alterations in the content and distribution of cytoskeleton structures , particularly actin microfilaments and microtubules .
	manualset3
105681	3	401729	13	NULL	NULL	0	NULL	content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been shown that viruses can induce alterations in the content and distribution of cytoskeleton structures , particularly actin microfilaments and microtubules .
	manualset3
105682	4	401729	13	NULL	NULL	0	NULL	distribution 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been shown that viruses can induce alterations in the content and distribution of cytoskeleton structures , particularly actin microfilaments and microtubules .
	manualset3
105683	5	401729	13	NULL	NULL	0	NULL	cytoskeleton structures	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been shown that viruses can induce alterations in the content and distribution of cytoskeleton structures , particularly actin microfilaments and microtubules .
	manualset3
105684	6	401729	13	NULL	NULL	0	NULL	actin microfilaments 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been shown that viruses can induce alterations in the content and distribution of cytoskeleton structures , particularly actin microfilaments and microtubules .
	manualset3
105685	7	401729	13	NULL	NULL	0	NULL	microtubules 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been shown that viruses can induce alterations in the content and distribution of cytoskeleton structures , particularly actin microfilaments and microtubules .
	manualset3
105686	1	401730	13	NULL	NULL	0	NULL	528IgG 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	528IgG , an anti-EGF-R murine monoclonal antibody and a polyclonal anti-EGF antibody were employed for immunostaining using the avidin-biotin method .
	manualset3
105687	2	401730	13	NULL	NULL	0	NULL	anti-EGF-R murine monoclonal antibody 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	528IgG , an anti-EGF-R murine monoclonal antibody and a polyclonal anti-EGF antibody were employed for immunostaining using the avidin-biotin method .
	manualset3
105688	3	401730	13	NULL	NULL	0	NULL	polyclonal anti-EGF antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	528IgG , an anti-EGF-R murine monoclonal antibody and a polyclonal anti-EGF antibody were employed for immunostaining using the avidin-biotin method .
	manualset3
105689	4	401730	13	NULL	NULL	0	NULL	immunostaining	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	528IgG , an anti-EGF-R murine monoclonal antibody and a polyclonal anti-EGF antibody were employed for immunostaining using the avidin-biotin method .
	manualset3
105690	5	401730	13	NULL	NULL	0	NULL	avidin-biotin method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	528IgG , an anti-EGF-R murine monoclonal antibody and a polyclonal anti-EGF antibody were employed for immunostaining using the avidin-biotin method .
	manualset3
105691	1	401731	13	NULL	NULL	0	NULL	fish	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been suggested that , in the fish , the change of otolith mass during development under altered gravity conditions and the growth of otoliths in normal conditions , are determined by feedback between otolith dynamics and the processes that regulate otolith growth .
	manualset3
105692	2	401731	13	NULL	NULL	0	NULL	change of otolith mass 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been suggested that , in the fish , the change of otolith mass during development under altered gravity conditions and the growth of otoliths in normal conditions , are determined by feedback between otolith dynamics and the processes that regulate otolith growth .
	manualset3
105693	3	401731	13	NULL	NULL	0	NULL	development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been suggested that , in the fish , the change of otolith mass during development under altered gravity conditions and the growth of otoliths in normal conditions , are determined by feedback between otolith dynamics and the processes that regulate otolith growth .
	manualset3
105694	4	401731	13	NULL	NULL	NULL	NULL	gravity conditions	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It has been suggested that , in the fish , the change of otolith mass during development under altered gravity conditions and the growth of otoliths in normal conditions , are determined by feedback between otolith dynamics and the processes that regulate otolith growth .
	manualset3
105695	5	401731	13	NULL	NULL	0	NULL	growth of otoliths	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been suggested that , in the fish , the change of otolith mass during development under altered gravity conditions and the growth of otoliths in normal conditions , are determined by feedback between otolith dynamics and the processes that regulate otolith growth .
	manualset3
105696	6	401731	13	NULL	NULL	0	NULL	normal conditions	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been suggested that , in the fish , the change of otolith mass during development under altered gravity conditions and the growth of otoliths in normal conditions , are determined by feedback between otolith dynamics and the processes that regulate otolith growth .
	manualset3
105697	7	401731	13	NULL	NULL	0	NULL	feedback 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been suggested that , in the fish , the change of otolith mass during development under altered gravity conditions and the growth of otoliths in normal conditions , are determined by feedback between otolith dynamics and the processes that regulate otolith growth .
	manualset3
105698	8	401731	13	NULL	NULL	0	NULL	otolith dynamics	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been suggested that , in the fish , the change of otolith mass during development under altered gravity conditions and the growth of otoliths in normal conditions , are determined by feedback between otolith dynamics and the processes that regulate otolith growth .
	manualset3
105699	9	401731	13	NULL	NULL	0	NULL	 processes 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been suggested that , in the fish , the change of otolith mass during development under altered gravity conditions and the growth of otoliths in normal conditions , are determined by feedback between otolith dynamics and the processes that regulate otolith growth .
	manualset3
105700	10	401731	13	NULL	NULL	0	NULL	 otolith growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been suggested that , in the fish , the change of otolith mass during development under altered gravity conditions and the growth of otoliths in normal conditions , are determined by feedback between otolith dynamics and the processes that regulate otolith growth .
	manualset3
105701	1	401732	13	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been suggested that genes involved in dopamine neurotransmission contribute to the pathogenesis of schizophrenia .
	manualset3
105702	2	401732	13	NULL	NULL	0	NULL	dopamine neurotransmission	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been suggested that genes involved in dopamine neurotransmission contribute to the pathogenesis of schizophrenia .
	manualset3
105703	3	401732	13	NULL	NULL	0	NULL	pathogenesis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been suggested that genes involved in dopamine neurotransmission contribute to the pathogenesis of schizophrenia .
	manualset3
105704	4	401732	13	NULL	NULL	0	NULL	schizophrenia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been suggested that genes involved in dopamine neurotransmission contribute to the pathogenesis of schizophrenia .
	manualset3
105705	1	401733	13	NULL	NULL	0	NULL	experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been suggested that increased training and experience may provide attention resource savings that can benefit the driver in handling new or unexpected traffic situations .
	manualset3
105707	3	401733	13	NULL	NULL	NULL	NULL	attention resource savings	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It has been suggested that increased training and experience may provide attention resource savings that can benefit the driver in handling new or unexpected traffic situations .
	manualset3
105708	4	401733	13	NULL	NULL	0	NULL	driver	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been suggested that increased training and experience may provide attention resource savings that can benefit the driver in handling new or unexpected traffic situations .
	manualset3
105709	5	401733	13	NULL	NULL	0	NULL	handling 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been suggested that increased training and experience may provide attention resource savings that can benefit the driver in handling new or unexpected traffic situations .
	manualset3
105710	6	401733	13	NULL	NULL	0	NULL	traffic situations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been suggested that increased training and experience may provide attention resource savings that can benefit the driver in handling new or unexpected traffic situations .
	manualset3
105711	1	401734	13	NULL	NULL	0	NULL	contralateral soft tissue defects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been used successfully to resurface contralateral soft tissue defects over the fingers , thumb and dorsum of the hand in eight cases .
	manualset3
105712	2	401734	13	NULL	NULL	0	NULL	fingers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been used successfully to resurface contralateral soft tissue defects over the fingers , thumb and dorsum of the hand in eight cases .
	manualset3
105713	3	401734	13	NULL	NULL	0	NULL	 thumb	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been used successfully to resurface contralateral soft tissue defects over the fingers , thumb and dorsum of the hand in eight cases .
	manualset3
105714	4	401734	13	NULL	NULL	0	NULL	 dorsum of the hand	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been used successfully to resurface contralateral soft tissue defects over the fingers , thumb and dorsum of the hand in eight cases .
	manualset3
105715	5	401734	13	NULL	NULL	0	NULL	eight cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been used successfully to resurface contralateral soft tissue defects over the fingers , thumb and dorsum of the hand in eight cases .
	manualset3
105716	1	401735	13	NULL	NULL	0	NULL	CT findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It has characteristic CT findings including a hemispheric cleft , either unilateral or bilateral , in the parasylvian region lined with heterotopic gray matter and extending from the pial to the ependymal surface .
	manualset3
105717	2	401735	13	NULL	NULL	0	NULL	hemispheric cleft	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It has characteristic CT findings including a hemispheric cleft , either unilateral or bilateral , in the parasylvian region lined with heterotopic gray matter and extending from the pial to the ependymal surface .
	manualset3
105718	3	401735	13	NULL	NULL	NULL	NULL	parasylvian region	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It has characteristic CT findings including a hemispheric cleft , either unilateral or bilateral , in the parasylvian region lined with heterotopic gray matter and extending from the pial to the ependymal surface .
	manualset3
105719	4	401735	13	NULL	NULL	0	NULL	heterotopic gray matter	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It has characteristic CT findings including a hemispheric cleft , either unilateral or bilateral , in the parasylvian region lined with heterotopic gray matter and extending from the pial to the ependymal surface .
	manualset3
105720	5	401735	13	NULL	NULL	0	NULL	ependymal surface	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It has characteristic CT findings including a hemispheric cleft , either unilateral or bilateral , in the parasylvian region lined with heterotopic gray matter and extending from the pial to the ependymal surface .
	manualset3
108305	6	401735	13	NULL	NULL	0	NULL	pial surface	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It has characteristic CT findings including a hemispheric cleft , either unilateral or bilateral , in the parasylvian region lined with heterotopic gray matter and extending from the pial to the ependymal surface .
	manualset3
105721	1	401736	13	NULL	NULL	0	NULL	 tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	It has developed in the tissues of multicellular organisms , both vertebrates and invertebrates , as a defense system to confine and eliminate foreign matter and , in this manner , protect the host against infection .
	manualset3
105722	2	401736	13	NULL	NULL	0	NULL	 multicellular organisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It has developed in the tissues of multicellular organisms , both vertebrates and invertebrates , as a defense system to confine and eliminate foreign matter and , in this manner , protect the host against infection .
	manualset3
105723	3	401736	13	NULL	NULL	0	NULL	vertebrates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It has developed in the tissues of multicellular organisms , both vertebrates and invertebrates , as a defense system to confine and eliminate foreign matter and , in this manner , protect the host against infection .
	manualset3
105724	4	401736	13	NULL	NULL	0	NULL	invertebrates 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It has developed in the tissues of multicellular organisms , both vertebrates and invertebrates , as a defense system to confine and eliminate foreign matter and , in this manner , protect the host against infection .
	manualset3
105725	5	401736	13	NULL	NULL	0	NULL	defense system	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It has developed in the tissues of multicellular organisms , both vertebrates and invertebrates , as a defense system to confine and eliminate foreign matter and , in this manner , protect the host against infection .
	manualset3
105726	6	401736	13	NULL	NULL	0	NULL	foreign matter	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	It has developed in the tissues of multicellular organisms , both vertebrates and invertebrates , as a defense system to confine and eliminate foreign matter and , in this manner , protect the host against infection .
	manualset3
105727	7	401736	13	NULL	NULL	0	NULL	manner	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It has developed in the tissues of multicellular organisms , both vertebrates and invertebrates , as a defense system to confine and eliminate foreign matter and , in this manner , protect the host against infection .
	manualset3
105728	8	401736	13	NULL	NULL	0	NULL	host 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It has developed in the tissues of multicellular organisms , both vertebrates and invertebrates , as a defense system to confine and eliminate foreign matter and , in this manner , protect the host against infection .
	manualset3
105729	9	401736	13	NULL	NULL	0	NULL	infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It has developed in the tissues of multicellular organisms , both vertebrates and invertebrates , as a defense system to confine and eliminate foreign matter and , in this manner , protect the host against infection .
	manualset3
105730	1	401737	13	NULL	NULL	0	NULL	homology 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	It has greatest homology with glucagon ( 48 % ) and human glucagon-like peptide-1 ( 50 % ) .
	manualset3
105731	2	401737	13	NULL	NULL	0	NULL	glucagon 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	It has greatest homology with glucagon ( 48 % ) and human glucagon-like peptide-1 ( 50 % ) .
	manualset3
105732	3	401737	13	NULL	NULL	0	NULL	 48 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It has greatest homology with glucagon ( 48 % ) and human glucagon-like peptide-1 ( 50 % ) .
	manualset3
105733	4	401737	13	NULL	NULL	0	NULL	human glucagon-like peptide-1	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	It has greatest homology with glucagon ( 48 % ) and human glucagon-like peptide-1 ( 50 % ) .
	manualset3
105734	5	401737	13	NULL	NULL	0	NULL	 50 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It has greatest homology with glucagon ( 48 % ) and human glucagon-like peptide-1 ( 50 % ) .
	manualset3
105735	1	401738	13	NULL	NULL	0	NULL	curative surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It has never been reported any radical curative surgery in presence of synchronous hepatic metastasis .
	manualset3
105736	2	401738	13	NULL	NULL	0	NULL	presence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It has never been reported any radical curative surgery in presence of synchronous hepatic metastasis .
	manualset3
105737	3	401738	13	NULL	NULL	0	NULL	synchronous hepatic metastasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It has never been reported any radical curative surgery in presence of synchronous hepatic metastasis .
	manualset3
105738	1	401739	13	NULL	NULL	0	NULL	CD43 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It has previously been shown that CD43 expression is altered in patients with myelodysplastic syndrome ( MDS ) .
	manualset3
105739	2	401739	13	NULL	NULL	0	NULL	 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It has previously been shown that CD43 expression is altered in patients with myelodysplastic syndrome ( MDS ) .
	manualset3
105740	3	401739	13	NULL	NULL	0	NULL	myelodysplastic syndrome ( MDS ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It has previously been shown that CD43 expression is altered in patients with myelodysplastic syndrome ( MDS ) .
	manualset3
105741	1	401740	13	NULL	NULL	0	NULL	 Notch	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It has recently been postulated that Notch instructively drives astrocyte differentiation .
	manualset3
105742	2	401740	13	NULL	NULL	0	NULL	astrocyte	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It has recently been postulated that Notch instructively drives astrocyte differentiation .
	manualset3
105743	3	401740	13	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It has recently been postulated that Notch instructively drives astrocyte differentiation .
	manualset3
105744	1	401741	13	NULL	NULL	0	NULL	functional groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It has shown that functional groups on C-829 or C-283 are , when the acridine portion of the molecule is intercalated as in a proflavine dinucleoside phosphate complex , in positions suitable for DNA cross-linking by activated 1-nitro-9-aminoacridine derivatives .
	manualset3
105745	2	401741	13	NULL	NULL	0	NULL	C-829 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It has shown that functional groups on C-829 or C-283 are , when the acridine portion of the molecule is intercalated as in a proflavine dinucleoside phosphate complex , in positions suitable for DNA cross-linking by activated 1-nitro-9-aminoacridine derivatives .
	manualset3
105746	3	401741	13	NULL	NULL	0	NULL	 C-283	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It has shown that functional groups on C-829 or C-283 are , when the acridine portion of the molecule is intercalated as in a proflavine dinucleoside phosphate complex , in positions suitable for DNA cross-linking by activated 1-nitro-9-aminoacridine derivatives .
	manualset3
105747	4	401741	13	NULL	NULL	0	NULL	acridine portion	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It has shown that functional groups on C-829 or C-283 are , when the acridine portion of the molecule is intercalated as in a proflavine dinucleoside phosphate complex , in positions suitable for DNA cross-linking by activated 1-nitro-9-aminoacridine derivatives .
	manualset3
105748	5	401741	13	NULL	NULL	0	NULL	molecule 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	It has shown that functional groups on C-829 or C-283 are , when the acridine portion of the molecule is intercalated as in a proflavine dinucleoside phosphate complex , in positions suitable for DNA cross-linking by activated 1-nitro-9-aminoacridine derivatives .
	manualset3
105749	6	401741	13	NULL	NULL	0	NULL	proflavine dinucleoside phosphate complex	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It has shown that functional groups on C-829 or C-283 are , when the acridine portion of the molecule is intercalated as in a proflavine dinucleoside phosphate complex , in positions suitable for DNA cross-linking by activated 1-nitro-9-aminoacridine derivatives .
	manualset3
105750	7	401741	13	NULL	NULL	0	NULL	positions 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It has shown that functional groups on C-829 or C-283 are , when the acridine portion of the molecule is intercalated as in a proflavine dinucleoside phosphate complex , in positions suitable for DNA cross-linking by activated 1-nitro-9-aminoacridine derivatives .
	manualset3
105751	8	401741	13	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It has shown that functional groups on C-829 or C-283 are , when the acridine portion of the molecule is intercalated as in a proflavine dinucleoside phosphate complex , in positions suitable for DNA cross-linking by activated 1-nitro-9-aminoacridine derivatives .
	manualset3
105752	9	401741	13	NULL	NULL	0	NULL	 1-nitro-9-aminoacridine derivatives	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It has shown that functional groups on C-829 or C-283 are , when the acridine portion of the molecule is intercalated as in a proflavine dinucleoside phosphate complex , in positions suitable for DNA cross-linking by activated 1-nitro-9-aminoacridine derivatives .
	manualset3
105753	1	401742	13	NULL	NULL	0	NULL	novel function 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It identifies a novel function for the MARV VP40 protein and suggests that MARV may globally inhibit Jak1-dependent cytokine signaling .
	manualset3
105754	2	401742	13	NULL	NULL	0	NULL	 MARV VP40 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It identifies a novel function for the MARV VP40 protein and suggests that MARV may globally inhibit Jak1-dependent cytokine signaling .
	manualset3
105755	3	401742	13	NULL	NULL	0	NULL	MARV	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It identifies a novel function for the MARV VP40 protein and suggests that MARV may globally inhibit Jak1-dependent cytokine signaling .
	manualset3
105756	4	401742	13	NULL	NULL	0	NULL	Jak1-dependent cytokine signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It identifies a novel function for the MARV VP40 protein and suggests that MARV may globally inhibit Jak1-dependent cytokine signaling .
	manualset3
105757	1	401743	13	NULL	NULL	0	NULL	 peritoneum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It implicate peritoneum , ovary 's surface and pelvis .
	manualset3
105758	2	401743	13	NULL	NULL	0	NULL	ovary 's surface 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It implicate peritoneum , ovary 's surface and pelvis .
	manualset3
105759	3	401743	13	NULL	NULL	0	NULL	pelvis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It implicate peritoneum , ovary 's surface and pelvis .
	manualset3
105760	1	401744	13	NULL	NULL	0	NULL	chronic osteomyelitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It includes chronic osteomyelitis as a sequel to late acute osteomyelitis as well as chronic unifocal and chronic multifocal osteomyelitis .
	manualset3
105761	2	401744	13	NULL	NULL	0	NULL	sequel	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It includes chronic osteomyelitis as a sequel to late acute osteomyelitis as well as chronic unifocal and chronic multifocal osteomyelitis .
	manualset3
105762	3	401744	13	NULL	NULL	0	NULL	late acute osteomyelitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It includes chronic osteomyelitis as a sequel to late acute osteomyelitis as well as chronic unifocal and chronic multifocal osteomyelitis .
	manualset3
105763	4	401744	13	NULL	NULL	0	NULL	chronic unifocal osteomyelitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It includes chronic osteomyelitis as a sequel to late acute osteomyelitis as well as chronic unifocal and chronic multifocal osteomyelitis .
	manualset3
105764	5	401744	13	NULL	NULL	0	NULL	chronic multifocal osteomyelitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It includes chronic osteomyelitis as a sequel to late acute osteomyelitis as well as chronic unifocal and chronic multifocal osteomyelitis .
	manualset3
105765	1	401745	13	NULL	NULL	0	NULL	medical care costs	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It includes medical care costs , household and wage work losses , and the value of pain , suffering , and lost quality of life .
	manualset3
105766	2	401745	13	NULL	NULL	0	NULL	household losses 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It includes medical care costs , household and wage work losses , and the value of pain , suffering , and lost quality of life .
	manualset3
105767	3	401745	13	NULL	NULL	0	NULL	wage work losses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It includes medical care costs , household and wage work losses , and the value of pain , suffering , and lost quality of life .
	manualset3
105768	4	401745	13	NULL	NULL	0	NULL	value of pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It includes medical care costs , household and wage work losses , and the value of pain , suffering , and lost quality of life .
	manualset3
105769	5	401745	13	NULL	NULL	0	NULL	 suffering	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It includes medical care costs , household and wage work losses , and the value of pain , suffering , and lost quality of life .
	manualset3
105770	6	401745	13	NULL	NULL	0	NULL	quality of life 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It includes medical care costs , household and wage work losses , and the value of pain , suffering , and lost quality of life .
	manualset3
105771	1	401746	13	NULL	NULL	0	NULL	 hard tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	It involves not only the hard tissues of the face , but the soft tissues as well .
	manualset3
105772	2	401746	13	NULL	NULL	0	NULL	face	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It involves not only the hard tissues of the face , but the soft tissues as well .
	manualset3
105773	3	401746	13	NULL	NULL	0	NULL	soft tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	It involves not only the hard tissues of the face , but the soft tissues as well .
	manualset3
105774	1	401747	13	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is a combination of flotation and rapid sand filtration , both of those being placed in the same tank .
	manualset3
105775	2	401747	13	NULL	NULL	0	NULL	flotation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is a combination of flotation and rapid sand filtration , both of those being placed in the same tank .
	manualset3
105776	3	401747	13	NULL	NULL	0	NULL	rapid sand filtration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is a combination of flotation and rapid sand filtration , both of those being placed in the same tank .
	manualset3
105777	4	401747	13	NULL	NULL	0	NULL	tank	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It is a combination of flotation and rapid sand filtration , both of those being placed in the same tank .
	manualset3
105778	1	401748	13	NULL	NULL	0	NULL	56 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	56 % of the patients reported using two types of asthma medicine .
	manualset3
105779	2	401748	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	56 % of the patients reported using two types of asthma medicine .
	manualset3
105780	3	401748	13	NULL	NULL	0	NULL	two types	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	56 % of the patients reported using two types of asthma medicine .
	manualset3
105781	4	401748	13	NULL	NULL	0	NULL	asthma medicine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	56 % of the patients reported using two types of asthma medicine .
	manualset3
105782	1	401749	13	NULL	NULL	NULL	NULL	stress 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is acknowledged that stress modulates gastrointestinal ( GI ) motility through central mechanisms including corticotropin-releasing-factor .
	manualset3
105783	2	401749	13	NULL	NULL	0	NULL	gastrointestinal ( GI ) motility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is acknowledged that stress modulates gastrointestinal ( GI ) motility through central mechanisms including corticotropin-releasing-factor .
	manualset3
105784	3	401749	13	NULL	NULL	0	NULL	central mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is acknowledged that stress modulates gastrointestinal ( GI ) motility through central mechanisms including corticotropin-releasing-factor .
	manualset3
105785	4	401749	13	NULL	NULL	0	NULL	corticotropin-releasing-factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is acknowledged that stress modulates gastrointestinal ( GI ) motility through central mechanisms including corticotropin-releasing-factor .
	manualset3
105786	1	401750	13	NULL	NULL	0	NULL	prostate cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It is also apparent that prostate cancer is now being detected at less advanced stages than in the past .
	manualset3
105787	2	401750	13	NULL	NULL	0	NULL	stages	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is also apparent that prostate cancer is now being detected at less advanced stages than in the past .
	manualset3
105788	3	401750	13	NULL	NULL	0	NULL	past	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	It is also apparent that prostate cancer is now being detected at less advanced stages than in the past .
	manualset3
105789	1	401751	13	NULL	NULL	0	NULL	family	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is also great family and social problem .
	manualset3
105790	2	401751	13	NULL	NULL	0	NULL	social problem	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is also great family and social problem .
	manualset3
105791	1	401752	13	NULL	NULL	0	NULL	human MAP three kinase 1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is also identical with the recently cloned human MAP three kinase 1 except for the lack of an internal sequence homologous to the murine MEKK-4alpha isoform .
	manualset3
105792	2	401752	13	NULL	NULL	0	NULL	lack 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is also identical with the recently cloned human MAP three kinase 1 except for the lack of an internal sequence homologous to the murine MEKK-4alpha isoform .
	manualset3
105793	3	401752	13	NULL	NULL	NULL	NULL	internal sequence	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is also identical with the recently cloned human MAP three kinase 1 except for the lack of an internal sequence homologous to the murine MEKK-4alpha isoform .
	manualset3
105794	4	401752	13	NULL	NULL	0	NULL	 murine MEKK-4alpha isoform 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is also identical with the recently cloned human MAP three kinase 1 except for the lack of an internal sequence homologous to the murine MEKK-4alpha isoform .
	manualset3
105795	1	401753	13	NULL	NULL	0	NULL	experience 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is also our experience that if Strongyloides colitis is included in the differential diagnosis , the correct diagnosis can usually be made .
	manualset3
105796	2	401753	13	NULL	NULL	0	NULL	Strongyloides colitis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It is also our experience that if Strongyloides colitis is included in the differential diagnosis , the correct diagnosis can usually be made .
	manualset3
105797	3	401753	13	NULL	NULL	0	NULL	differential diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is also our experience that if Strongyloides colitis is included in the differential diagnosis , the correct diagnosis can usually be made .
	manualset3
105798	4	401753	13	NULL	NULL	0	NULL	correct diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is also our experience that if Strongyloides colitis is included in the differential diagnosis , the correct diagnosis can usually be made .
	manualset3
105799	1	401754	13	NULL	NULL	0	NULL	conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	It is also suggested that , in those conditions that lead to an inordinate accumulation of Ca2 + into myocardial cells , the unmatched demands of energy and the depletion of ATP play a primary role in the irreversible stage of cell damage .
	manualset3
105800	2	401754	13	NULL	NULL	0	NULL	accumulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is also suggested that , in those conditions that lead to an inordinate accumulation of Ca2 + into myocardial cells , the unmatched demands of energy and the depletion of ATP play a primary role in the irreversible stage of cell damage .
	manualset3
105801	3	401754	13	NULL	NULL	0	NULL	Ca2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	It is also suggested that , in those conditions that lead to an inordinate accumulation of Ca2 + into myocardial cells , the unmatched demands of energy and the depletion of ATP play a primary role in the irreversible stage of cell damage .
	manualset3
105802	4	401754	13	NULL	NULL	0	NULL	myocardial cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It is also suggested that , in those conditions that lead to an inordinate accumulation of Ca2 + into myocardial cells , the unmatched demands of energy and the depletion of ATP play a primary role in the irreversible stage of cell damage .
	manualset3
105803	5	401754	13	NULL	NULL	0	NULL	energy	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is also suggested that , in those conditions that lead to an inordinate accumulation of Ca2 + into myocardial cells , the unmatched demands of energy and the depletion of ATP play a primary role in the irreversible stage of cell damage .
	manualset3
105804	6	401754	13	NULL	NULL	0	NULL	depletion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is also suggested that , in those conditions that lead to an inordinate accumulation of Ca2 + into myocardial cells , the unmatched demands of energy and the depletion of ATP play a primary role in the irreversible stage of cell damage .
	manualset3
105805	7	401754	13	NULL	NULL	0	NULL	ATP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	It is also suggested that , in those conditions that lead to an inordinate accumulation of Ca2 + into myocardial cells , the unmatched demands of energy and the depletion of ATP play a primary role in the irreversible stage of cell damage .
	manualset3
105806	8	401754	13	NULL	NULL	NULL	NULL	play 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is also suggested that , in those conditions that lead to an inordinate accumulation of Ca2 + into myocardial cells , the unmatched demands of energy and the depletion of ATP play a primary role in the irreversible stage of cell damage .
	manualset3
105807	9	401754	13	NULL	NULL	0	NULL	role 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is also suggested that , in those conditions that lead to an inordinate accumulation of Ca2 + into myocardial cells , the unmatched demands of energy and the depletion of ATP play a primary role in the irreversible stage of cell damage .
	manualset3
105808	10	401754	13	NULL	NULL	0	NULL	stage	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	It is also suggested that , in those conditions that lead to an inordinate accumulation of Ca2 + into myocardial cells , the unmatched demands of energy and the depletion of ATP play a primary role in the irreversible stage of cell damage .
	manualset3
105809	11	401754	13	NULL	NULL	0	NULL	cell damage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is also suggested that , in those conditions that lead to an inordinate accumulation of Ca2 + into myocardial cells , the unmatched demands of energy and the depletion of ATP play a primary role in the irreversible stage of cell damage .
	manualset3
105810	1	401755	13	NULL	NULL	0	NULL	absence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is argued that absence of Cr causes the higher relative P ( i ) concentration also observed in animals lacking muscle CK , indicating an important role of the CK system in P ( i ) homeostasis .
	manualset3
105811	2	401755	13	NULL	NULL	0	NULL	 Cr 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	It is argued that absence of Cr causes the higher relative P ( i ) concentration also observed in animals lacking muscle CK , indicating an important role of the CK system in P ( i ) homeostasis .
	manualset3
105812	3	401755	13	NULL	NULL	0	NULL	P ( i ) concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is argued that absence of Cr causes the higher relative P ( i ) concentration also observed in animals lacking muscle CK , indicating an important role of the CK system in P ( i ) homeostasis .
	manualset3
105813	4	401755	13	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It is argued that absence of Cr causes the higher relative P ( i ) concentration also observed in animals lacking muscle CK , indicating an important role of the CK system in P ( i ) homeostasis .
	manualset3
105814	5	401755	13	NULL	NULL	0	NULL	muscle CK 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is argued that absence of Cr causes the higher relative P ( i ) concentration also observed in animals lacking muscle CK , indicating an important role of the CK system in P ( i ) homeostasis .
	manualset3
105815	6	401755	13	NULL	NULL	0	NULL	 role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is argued that absence of Cr causes the higher relative P ( i ) concentration also observed in animals lacking muscle CK , indicating an important role of the CK system in P ( i ) homeostasis .
	manualset3
105816	7	401755	13	NULL	NULL	0	NULL	CK system	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is argued that absence of Cr causes the higher relative P ( i ) concentration also observed in animals lacking muscle CK , indicating an important role of the CK system in P ( i ) homeostasis .
	manualset3
105817	8	401755	13	NULL	NULL	0	NULL	P ( i ) homeostasis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is argued that absence of Cr causes the higher relative P ( i ) concentration also observed in animals lacking muscle CK , indicating an important role of the CK system in P ( i ) homeostasis .
	manualset3
105818	1	401756	13	NULL	NULL	NULL	NULL	continuity 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is argued that decontextualized continuity tends to occur within a given lifestage , whereas contextualized change is apt to emerge during a transition from one lifestage to another .
	manualset3
105819	2	401756	13	NULL	NULL	0	NULL	lifestage	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	It is argued that decontextualized continuity tends to occur within a given lifestage , whereas contextualized change is apt to emerge during a transition from one lifestage to another .
	manualset3
105820	3	401756	13	NULL	NULL	0	NULL	change	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is argued that decontextualized continuity tends to occur within a given lifestage , whereas contextualized change is apt to emerge during a transition from one lifestage to another .
	manualset3
105821	4	401756	13	NULL	NULL	0	NULL	transition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is argued that decontextualized continuity tends to occur within a given lifestage , whereas contextualized change is apt to emerge during a transition from one lifestage to another .
	manualset3
105822	5	401756	13	NULL	NULL	0	NULL	lifestage	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	It is argued that decontextualized continuity tends to occur within a given lifestage , whereas contextualized change is apt to emerge during a transition from one lifestage to another .
	manualset3
105823	1	401757	13	NULL	NULL	0	NULL	situations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is argued that for both situations the dominant contributions to the dissipative part of the dynamics arise from the excitation of electron-hole pairs and from the subsequent relaxation of these pairs by spin-dependent scattering processes , which transfer angular momentum to the lattice .
	manualset3
105824	2	401757	13	NULL	NULL	0	NULL	dominant contributions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is argued that for both situations the dominant contributions to the dissipative part of the dynamics arise from the excitation of electron-hole pairs and from the subsequent relaxation of these pairs by spin-dependent scattering processes , which transfer angular momentum to the lattice .
	manualset3
105825	3	401757	13	NULL	NULL	0	NULL	dissipative part 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is argued that for both situations the dominant contributions to the dissipative part of the dynamics arise from the excitation of electron-hole pairs and from the subsequent relaxation of these pairs by spin-dependent scattering processes , which transfer angular momentum to the lattice .
	manualset3
105826	4	401757	13	NULL	NULL	0	NULL	 dynamics 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is argued that for both situations the dominant contributions to the dissipative part of the dynamics arise from the excitation of electron-hole pairs and from the subsequent relaxation of these pairs by spin-dependent scattering processes , which transfer angular momentum to the lattice .
	manualset3
105827	5	401757	13	NULL	NULL	0	NULL	excitation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is argued that for both situations the dominant contributions to the dissipative part of the dynamics arise from the excitation of electron-hole pairs and from the subsequent relaxation of these pairs by spin-dependent scattering processes , which transfer angular momentum to the lattice .
	manualset3
105828	6	401757	13	NULL	NULL	NULL	NULL	electron-hole pairs	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is argued that for both situations the dominant contributions to the dissipative part of the dynamics arise from the excitation of electron-hole pairs and from the subsequent relaxation of these pairs by spin-dependent scattering processes , which transfer angular momentum to the lattice .
	manualset3
105829	7	401757	13	NULL	NULL	0	NULL	relaxation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is argued that for both situations the dominant contributions to the dissipative part of the dynamics arise from the excitation of electron-hole pairs and from the subsequent relaxation of these pairs by spin-dependent scattering processes , which transfer angular momentum to the lattice .
	manualset3
105830	8	401757	13	NULL	NULL	0	NULL	pairs 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It is argued that for both situations the dominant contributions to the dissipative part of the dynamics arise from the excitation of electron-hole pairs and from the subsequent relaxation of these pairs by spin-dependent scattering processes , which transfer angular momentum to the lattice .
	manualset3
105831	9	401757	13	NULL	NULL	0	NULL	spin-dependent scattering processes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is argued that for both situations the dominant contributions to the dissipative part of the dynamics arise from the excitation of electron-hole pairs and from the subsequent relaxation of these pairs by spin-dependent scattering processes , which transfer angular momentum to the lattice .
	manualset3
105832	10	401757	13	NULL	NULL	0	NULL	transfer	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is argued that for both situations the dominant contributions to the dissipative part of the dynamics arise from the excitation of electron-hole pairs and from the subsequent relaxation of these pairs by spin-dependent scattering processes , which transfer angular momentum to the lattice .
	manualset3
105833	11	401757	13	NULL	NULL	0	NULL	angular momentum	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is argued that for both situations the dominant contributions to the dissipative part of the dynamics arise from the excitation of electron-hole pairs and from the subsequent relaxation of these pairs by spin-dependent scattering processes , which transfer angular momentum to the lattice .
	manualset3
105834	12	401757	13	NULL	NULL	0	NULL	lattice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is argued that for both situations the dominant contributions to the dissipative part of the dynamics arise from the excitation of electron-hole pairs and from the subsequent relaxation of these pairs by spin-dependent scattering processes , which transfer angular momentum to the lattice .
	manualset3
105835	1	401758	13	NULL	NULL	0	NULL	chronic SCI	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is assumed that in chronic SCI the patient 's immobility results in a reduced input from supraspinal and peripheral sources and leads to a dominance of inhibitory drive within spinal neuronal circuitries underlying locomotor pattern and spinal reflex generation .
	manualset3
105836	2	401758	13	NULL	NULL	0	NULL	patient 's immobility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is assumed that in chronic SCI the patient 's immobility results in a reduced input from supraspinal and peripheral sources and leads to a dominance of inhibitory drive within spinal neuronal circuitries underlying locomotor pattern and spinal reflex generation .
	manualset3
105837	3	401758	13	NULL	NULL	0	NULL	results	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is assumed that in chronic SCI the patient 's immobility results in a reduced input from supraspinal and peripheral sources and leads to a dominance of inhibitory drive within spinal neuronal circuitries underlying locomotor pattern and spinal reflex generation .
	manualset3
105838	4	401758	13	NULL	NULL	0	NULL	input	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is assumed that in chronic SCI the patient 's immobility results in a reduced input from supraspinal and peripheral sources and leads to a dominance of inhibitory drive within spinal neuronal circuitries underlying locomotor pattern and spinal reflex generation .
	manualset3
105839	5	401758	13	NULL	NULL	0	NULL	supraspinal sources	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is assumed that in chronic SCI the patient 's immobility results in a reduced input from supraspinal and peripheral sources and leads to a dominance of inhibitory drive within spinal neuronal circuitries underlying locomotor pattern and spinal reflex generation .
	manualset3
105840	6	401758	13	NULL	NULL	0	NULL	peripheral sources	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is assumed that in chronic SCI the patient 's immobility results in a reduced input from supraspinal and peripheral sources and leads to a dominance of inhibitory drive within spinal neuronal circuitries underlying locomotor pattern and spinal reflex generation .
	manualset3
105841	7	401758	13	NULL	NULL	0	NULL	dominance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is assumed that in chronic SCI the patient 's immobility results in a reduced input from supraspinal and peripheral sources and leads to a dominance of inhibitory drive within spinal neuronal circuitries underlying locomotor pattern and spinal reflex generation .
	manualset3
105842	8	401758	13	NULL	NULL	0	NULL	inhibitory drive	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is assumed that in chronic SCI the patient 's immobility results in a reduced input from supraspinal and peripheral sources and leads to a dominance of inhibitory drive within spinal neuronal circuitries underlying locomotor pattern and spinal reflex generation .
	manualset3
105844	10	401758	13	NULL	NULL	0	NULL	locomotor pattern 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is assumed that in chronic SCI the patient 's immobility results in a reduced input from supraspinal and peripheral sources and leads to a dominance of inhibitory drive within spinal neuronal circuitries underlying locomotor pattern and spinal reflex generation .
	manualset3
105845	11	401758	13	NULL	NULL	0	NULL	spinal reflex generation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is assumed that in chronic SCI the patient 's immobility results in a reduced input from supraspinal and peripheral sources and leads to a dominance of inhibitory drive within spinal neuronal circuitries underlying locomotor pattern and spinal reflex generation .
	manualset3
105843	1	401759	13	NULL	NULL	NULL	NULL	mechanism	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is assumed that the mechanism that triggers the increase of the rate of MSM generation may lie in lipid peroxidation activation .
	manualset3
105846	2	401759	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is assumed that the mechanism that triggers the increase of the rate of MSM generation may lie in lipid peroxidation activation .
	manualset3
105847	3	401759	13	NULL	NULL	0	NULL	rate 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is assumed that the mechanism that triggers the increase of the rate of MSM generation may lie in lipid peroxidation activation .
	manualset3
105848	4	401759	13	NULL	NULL	0	NULL	MSM generation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is assumed that the mechanism that triggers the increase of the rate of MSM generation may lie in lipid peroxidation activation .
	manualset3
105849	5	401759	13	NULL	NULL	0	NULL	lipid peroxidation activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is assumed that the mechanism that triggers the increase of the rate of MSM generation may lie in lipid peroxidation activation .
	manualset3
105850	1	401760	13	NULL	NULL	0	NULL	division	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is based on a division of labor between doctor and midwife and demands an increasing number of consultations , vaginal control of the cervix in the period of advanced danger of premature delivery and includes a short psycho-prophylactic program .
	manualset3
105851	2	401760	13	NULL	NULL	0	NULL	labor	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is based on a division of labor between doctor and midwife and demands an increasing number of consultations , vaginal control of the cervix in the period of advanced danger of premature delivery and includes a short psycho-prophylactic program .
	manualset3
105852	3	401760	13	NULL	NULL	0	NULL	doctor 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	It is based on a division of labor between doctor and midwife and demands an increasing number of consultations , vaginal control of the cervix in the period of advanced danger of premature delivery and includes a short psycho-prophylactic program .
	manualset3
105853	4	401760	13	NULL	NULL	0	NULL	midwife 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	It is based on a division of labor between doctor and midwife and demands an increasing number of consultations , vaginal control of the cervix in the period of advanced danger of premature delivery and includes a short psycho-prophylactic program .
	manualset3
105854	5	401760	13	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It is based on a division of labor between doctor and midwife and demands an increasing number of consultations , vaginal control of the cervix in the period of advanced danger of premature delivery and includes a short psycho-prophylactic program .
	manualset3
105855	6	401760	13	NULL	NULL	0	NULL	consultations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is based on a division of labor between doctor and midwife and demands an increasing number of consultations , vaginal control of the cervix in the period of advanced danger of premature delivery and includes a short psycho-prophylactic program .
	manualset3
105856	7	401760	13	NULL	NULL	0	NULL	vaginal control of the cervix	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is based on a division of labor between doctor and midwife and demands an increasing number of consultations , vaginal control of the cervix in the period of advanced danger of premature delivery and includes a short psycho-prophylactic program .
	manualset3
105857	8	401760	13	NULL	NULL	0	NULL	period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	It is based on a division of labor between doctor and midwife and demands an increasing number of consultations , vaginal control of the cervix in the period of advanced danger of premature delivery and includes a short psycho-prophylactic program .
	manualset3
105858	9	401760	13	NULL	NULL	0	NULL	danger of premature delivery	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is based on a division of labor between doctor and midwife and demands an increasing number of consultations , vaginal control of the cervix in the period of advanced danger of premature delivery and includes a short psycho-prophylactic program .
	manualset3
105859	10	401760	13	NULL	NULL	0	NULL	short psycho-prophylactic program	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is based on a division of labor between doctor and midwife and demands an increasing number of consultations , vaginal control of the cervix in the period of advanced danger of premature delivery and includes a short psycho-prophylactic program .
	manualset3
105860	1	401761	13	NULL	NULL	0	NULL	finite element computer simulation model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	It is based on a previously developed finite element computer simulation model for laminar-separated flow in arteries of axially varying cross-section ; the present modification allows use of angiographic stenosis shapes acquired by automatic edge-detection algorithms .
	manualset3
105861	2	401761	13	NULL	NULL	0	NULL	laminar-separated flow	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is based on a previously developed finite element computer simulation model for laminar-separated flow in arteries of axially varying cross-section ; the present modification allows use of angiographic stenosis shapes acquired by automatic edge-detection algorithms .
	manualset3
105862	3	401761	13	NULL	NULL	0	NULL	arteries of axially varying cross-section	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is based on a previously developed finite element computer simulation model for laminar-separated flow in arteries of axially varying cross-section ; the present modification allows use of angiographic stenosis shapes acquired by automatic edge-detection algorithms .
	manualset3
105863	4	401761	13	NULL	NULL	0	NULL	modification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is based on a previously developed finite element computer simulation model for laminar-separated flow in arteries of axially varying cross-section ; the present modification allows use of angiographic stenosis shapes acquired by automatic edge-detection algorithms .
	manualset3
105864	5	401761	13	NULL	NULL	0	NULL	 use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is based on a previously developed finite element computer simulation model for laminar-separated flow in arteries of axially varying cross-section ; the present modification allows use of angiographic stenosis shapes acquired by automatic edge-detection algorithms .
	manualset3
105865	6	401761	13	NULL	NULL	0	NULL	angiographic stenosis shapes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is based on a previously developed finite element computer simulation model for laminar-separated flow in arteries of axially varying cross-section ; the present modification allows use of angiographic stenosis shapes acquired by automatic edge-detection algorithms .
	manualset3
105866	7	401761	13	NULL	NULL	0	NULL	automatic edge-detection algorithms	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	It is based on a previously developed finite element computer simulation model for laminar-separated flow in arteries of axially varying cross-section ; the present modification allows use of angiographic stenosis shapes acquired by automatic edge-detection algorithms .
	manualset3
105867	1	401762	13	NULL	NULL	0	NULL	 rotational modules	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is based on rotational modules with daily cycles of interactive , case-based small-group seminars , PBL tutorials and training of sensomotor and communication skills .
	manualset3
105868	2	401762	13	NULL	NULL	0	NULL	daily cycles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is based on rotational modules with daily cycles of interactive , case-based small-group seminars , PBL tutorials and training of sensomotor and communication skills .
	manualset3
105869	3	401762	13	NULL	NULL	0	NULL	case-based small-group seminars 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is based on rotational modules with daily cycles of interactive , case-based small-group seminars , PBL tutorials and training of sensomotor and communication skills .
	manualset3
105870	4	401762	13	NULL	NULL	0	NULL	PBL tutorials 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is based on rotational modules with daily cycles of interactive , case-based small-group seminars , PBL tutorials and training of sensomotor and communication skills .
	manualset3
105871	5	401762	13	NULL	NULL	0	NULL	training 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is based on rotational modules with daily cycles of interactive , case-based small-group seminars , PBL tutorials and training of sensomotor and communication skills .
	manualset3
105872	6	401762	13	NULL	NULL	0	NULL	sensomotor skills 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is based on rotational modules with daily cycles of interactive , case-based small-group seminars , PBL tutorials and training of sensomotor and communication skills .
	manualset3
105873	7	401762	13	NULL	NULL	0	NULL	communication skills	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is based on rotational modules with daily cycles of interactive , case-based small-group seminars , PBL tutorials and training of sensomotor and communication skills .
	manualset3
105874	1	401763	13	NULL	NULL	0	NULL	PCSK9 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is believed that PCSK9 binds to LDL-receptor ( LDLR ) protein and prevents its recycling to the cell surface ; gain-of-function PCSK9 mutants enhance LDLR degradation .
	manualset3
105875	2	401763	13	NULL	NULL	0	NULL	LDL-receptor ( LDLR ) protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is believed that PCSK9 binds to LDL-receptor ( LDLR ) protein and prevents its recycling to the cell surface ; gain-of-function PCSK9 mutants enhance LDLR degradation .
	manualset3
105876	3	401763	13	NULL	NULL	0	NULL	cell surface	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	It is believed that PCSK9 binds to LDL-receptor ( LDLR ) protein and prevents its recycling to the cell surface ; gain-of-function PCSK9 mutants enhance LDLR degradation .
	manualset3
105877	4	401763	13	NULL	NULL	0	NULL	gain-of-function 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is believed that PCSK9 binds to LDL-receptor ( LDLR ) protein and prevents its recycling to the cell surface ; gain-of-function PCSK9 mutants enhance LDLR degradation .
	manualset3
105878	5	401763	13	NULL	NULL	0	NULL	PCSK9 mutants 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is believed that PCSK9 binds to LDL-receptor ( LDLR ) protein and prevents its recycling to the cell surface ; gain-of-function PCSK9 mutants enhance LDLR degradation .
	manualset3
105879	6	401763	13	NULL	NULL	0	NULL	LDLR degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is believed that PCSK9 binds to LDL-receptor ( LDLR ) protein and prevents its recycling to the cell surface ; gain-of-function PCSK9 mutants enhance LDLR degradation .
	manualset3
105880	1	401764	13	NULL	NULL	NULL	NULL	6 ( - ) - Propranolol 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	6 ( - ) - Propranolol , guanethidine and CPA produced a short period of electrocortical desynchronization at the beginning of the perfusion period before antagonism of the amphetamine response was apparent .
	manualset3
105881	2	401764	13	NULL	NULL	0	NULL	 guanethidine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	6 ( - ) - Propranolol , guanethidine and CPA produced a short period of electrocortical desynchronization at the beginning of the perfusion period before antagonism of the amphetamine response was apparent .
	manualset3
105882	3	401764	13	NULL	NULL	0	NULL	CPA 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	6 ( - ) - Propranolol , guanethidine and CPA produced a short period of electrocortical desynchronization at the beginning of the perfusion period before antagonism of the amphetamine response was apparent .
	manualset3
105883	4	401764	13	NULL	NULL	0	NULL	short period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	6 ( - ) - Propranolol , guanethidine and CPA produced a short period of electrocortical desynchronization at the beginning of the perfusion period before antagonism of the amphetamine response was apparent .
	manualset3
105884	5	401764	13	NULL	NULL	0	NULL	electrocortical desynchronization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	6 ( - ) - Propranolol , guanethidine and CPA produced a short period of electrocortical desynchronization at the beginning of the perfusion period before antagonism of the amphetamine response was apparent .
	manualset3
105885	6	401764	13	NULL	NULL	0	NULL	beginning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	6 ( - ) - Propranolol , guanethidine and CPA produced a short period of electrocortical desynchronization at the beginning of the perfusion period before antagonism of the amphetamine response was apparent .
	manualset3
105886	7	401764	13	NULL	NULL	0	NULL	perfusion period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	6 ( - ) - Propranolol , guanethidine and CPA produced a short period of electrocortical desynchronization at the beginning of the perfusion period before antagonism of the amphetamine response was apparent .
	manualset3
105887	8	401764	13	NULL	NULL	0	NULL	antagonism 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	6 ( - ) - Propranolol , guanethidine and CPA produced a short period of electrocortical desynchronization at the beginning of the perfusion period before antagonism of the amphetamine response was apparent .
	manualset3
105888	9	401764	13	NULL	NULL	0	NULL	amphetamine response 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	6 ( - ) - Propranolol , guanethidine and CPA produced a short period of electrocortical desynchronization at the beginning of the perfusion period before antagonism of the amphetamine response was apparent .
	manualset3
105889	1	401765	13	NULL	NULL	0	NULL	treatment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is beneficial in the treatment of eclampsia , a disease with a pathophysiology comparable to DCI after subarachnoid hemorrhage .
	manualset3
105890	2	401765	13	NULL	NULL	0	NULL	eclampsia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It is beneficial in the treatment of eclampsia , a disease with a pathophysiology comparable to DCI after subarachnoid hemorrhage .
	manualset3
105891	3	401765	13	NULL	NULL	NULL	NULL	disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is beneficial in the treatment of eclampsia , a disease with a pathophysiology comparable to DCI after subarachnoid hemorrhage .
	manualset3
105892	4	401765	13	NULL	NULL	NULL	NULL	pathophysiology 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is beneficial in the treatment of eclampsia , a disease with a pathophysiology comparable to DCI after subarachnoid hemorrhage .
	manualset3
105893	5	401765	13	NULL	NULL	0	NULL	DCI 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is beneficial in the treatment of eclampsia , a disease with a pathophysiology comparable to DCI after subarachnoid hemorrhage .
	manualset3
105894	6	401765	13	NULL	NULL	0	NULL	 subarachnoid hemorrhage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is beneficial in the treatment of eclampsia , a disease with a pathophysiology comparable to DCI after subarachnoid hemorrhage .
	manualset3
105895	1	401766	13	NULL	NULL	0	NULL	majority of breast tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It is both overexpressed and aberrantly glycosylated in the majority of breast tumors , resulting in an antigenically distinct molecule and a potential target for immunotherapy trials .
	manualset3
105896	2	401766	13	NULL	NULL	0	NULL	molecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	It is both overexpressed and aberrantly glycosylated in the majority of breast tumors , resulting in an antigenically distinct molecule and a potential target for immunotherapy trials .
	manualset3
105897	3	401766	13	NULL	NULL	0	NULL	potential target	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is both overexpressed and aberrantly glycosylated in the majority of breast tumors , resulting in an antigenically distinct molecule and a potential target for immunotherapy trials .
	manualset3
105898	4	401766	13	NULL	NULL	0	NULL	immunotherapy trials 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is both overexpressed and aberrantly glycosylated in the majority of breast tumors , resulting in an antigenically distinct molecule and a potential target for immunotherapy trials .
	manualset3
105899	1	401767	13	NULL	NULL	NULL	NULL	sequence	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is closely related to the sequence of protein SCMKB-IIIB3 ( Haylett , Swart & Parris , 1971 ) differing in only four positions .
	manualset3
105900	2	401767	13	NULL	NULL	0	NULL	protein SCMKB-IIIB3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is closely related to the sequence of protein SCMKB-IIIB3 ( Haylett , Swart & Parris , 1971 ) differing in only four positions .
	manualset3
105901	3	401767	13	NULL	NULL	0	NULL	Haylett	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	It is closely related to the sequence of protein SCMKB-IIIB3 ( Haylett , Swart & Parris , 1971 ) differing in only four positions .
	manualset3
105902	4	401767	13	NULL	NULL	0	NULL	Swart	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	It is closely related to the sequence of protein SCMKB-IIIB3 ( Haylett , Swart & Parris , 1971 ) differing in only four positions .
	manualset3
105903	5	401767	13	NULL	NULL	0	NULL	Parris	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	It is closely related to the sequence of protein SCMKB-IIIB3 ( Haylett , Swart & Parris , 1971 ) differing in only four positions .
	manualset3
105904	6	401767	13	NULL	NULL	0	NULL	1971	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	It is closely related to the sequence of protein SCMKB-IIIB3 ( Haylett , Swart & Parris , 1971 ) differing in only four positions .
	manualset3
105905	7	401767	13	NULL	NULL	0	NULL	four positions	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It is closely related to the sequence of protein SCMKB-IIIB3 ( Haylett , Swart & Parris , 1971 ) differing in only four positions .
	manualset3
105906	1	401768	13	NULL	NULL	0	NULL	imaging techniques	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is complementary to other imaging techniques such as ultrasonography and scintigraphy .
	manualset3
105907	2	401768	13	NULL	NULL	0	NULL	ultrasonography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is complementary to other imaging techniques such as ultrasonography and scintigraphy .
	manualset3
105908	3	401768	13	NULL	NULL	0	NULL	scintigraphy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is complementary to other imaging techniques such as ultrasonography and scintigraphy .
	manualset3
105909	1	401769	13	NULL	NULL	0	NULL	 Fgfrl1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is conceivable that Fgfrl1 interacts with other Fgfrs , which are expressed in cartilage and muscle , to modulate FGF signaling .
	manualset3
105910	2	401769	13	NULL	NULL	0	NULL	Fgfrs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is conceivable that Fgfrl1 interacts with other Fgfrs , which are expressed in cartilage and muscle , to modulate FGF signaling .
	manualset3
105911	3	401769	13	NULL	NULL	0	NULL	cartilage	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	It is conceivable that Fgfrl1 interacts with other Fgfrs , which are expressed in cartilage and muscle , to modulate FGF signaling .
	manualset3
105912	4	401769	13	NULL	NULL	0	NULL	muscle	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	It is conceivable that Fgfrl1 interacts with other Fgfrs , which are expressed in cartilage and muscle , to modulate FGF signaling .
	manualset3
105913	5	401769	13	NULL	NULL	0	NULL	FGF signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is conceivable that Fgfrl1 interacts with other Fgfrs , which are expressed in cartilage and muscle , to modulate FGF signaling .
	manualset3
105914	1	401770	13	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded from the above results that if exercise-induced ST elevation at the infarcted area reflects transient myocardial ischemia , ISDN can decrease it by its anti-anginal effect .
	manualset3
105915	2	401770	13	NULL	NULL	0	NULL	exercise-induced ST elevation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded from the above results that if exercise-induced ST elevation at the infarcted area reflects transient myocardial ischemia , ISDN can decrease it by its anti-anginal effect .
	manualset3
105916	3	401770	13	NULL	NULL	0	NULL	area 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded from the above results that if exercise-induced ST elevation at the infarcted area reflects transient myocardial ischemia , ISDN can decrease it by its anti-anginal effect .
	manualset3
105917	4	401770	13	NULL	NULL	0	NULL	 transient myocardial ischemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded from the above results that if exercise-induced ST elevation at the infarcted area reflects transient myocardial ischemia , ISDN can decrease it by its anti-anginal effect .
	manualset3
105918	5	401770	13	NULL	NULL	0	NULL	ISDN 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded from the above results that if exercise-induced ST elevation at the infarcted area reflects transient myocardial ischemia , ISDN can decrease it by its anti-anginal effect .
	manualset3
105919	6	401770	13	NULL	NULL	0	NULL	anti-anginal effect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded from the above results that if exercise-induced ST elevation at the infarcted area reflects transient myocardial ischemia , ISDN can decrease it by its anti-anginal effect .
	manualset3
105934	1	401771	13	NULL	NULL	0	NULL	effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that , when the effect of protein deprivation on ATP sulphurylase is separated from the effect of vitamin A deficiency , a lowering of the enzyme activity caused by the vitamin deficiency is demonstrable .
	manualset3
105935	2	401771	13	NULL	NULL	0	NULL	protein deprivation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that , when the effect of protein deprivation on ATP sulphurylase is separated from the effect of vitamin A deficiency , a lowering of the enzyme activity caused by the vitamin deficiency is demonstrable .
	manualset3
105938	3	401771	13	NULL	NULL	0	NULL	ATP sulphurylase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that , when the effect of protein deprivation on ATP sulphurylase is separated from the effect of vitamin A deficiency , a lowering of the enzyme activity caused by the vitamin deficiency is demonstrable .
	manualset3
105941	4	401771	13	NULL	NULL	0	NULL	effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that , when the effect of protein deprivation on ATP sulphurylase is separated from the effect of vitamin A deficiency , a lowering of the enzyme activity caused by the vitamin deficiency is demonstrable .
	manualset3
105943	5	401771	13	NULL	NULL	0	NULL	vitamin A deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that , when the effect of protein deprivation on ATP sulphurylase is separated from the effect of vitamin A deficiency , a lowering of the enzyme activity caused by the vitamin deficiency is demonstrable .
	manualset3
105946	6	401771	13	NULL	NULL	0	NULL	enzyme activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that , when the effect of protein deprivation on ATP sulphurylase is separated from the effect of vitamin A deficiency , a lowering of the enzyme activity caused by the vitamin deficiency is demonstrable .
	manualset3
105949	7	401771	13	NULL	NULL	0	NULL	vitamin deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that , when the effect of protein deprivation on ATP sulphurylase is separated from the effect of vitamin A deficiency , a lowering of the enzyme activity caused by the vitamin deficiency is demonstrable .
	manualset3
105987	1	401772	13	NULL	NULL	0	NULL	Cyps	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that Cyps might play a role , probably as mediators in the pathophysiology of sepsis or as symptoms of diagnostic value .
	manualset3
105988	2	401772	13	NULL	NULL	0	NULL	role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that Cyps might play a role , probably as mediators in the pathophysiology of sepsis or as symptoms of diagnostic value .
	manualset3
105991	3	401772	13	NULL	NULL	NULL	NULL	mediators	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is concluded that Cyps might play a role , probably as mediators in the pathophysiology of sepsis or as symptoms of diagnostic value .
	manualset3
105994	4	401772	13	NULL	NULL	0	NULL	pathophysiology of sepsis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that Cyps might play a role , probably as mediators in the pathophysiology of sepsis or as symptoms of diagnostic value .
	manualset3
105995	5	401772	13	NULL	NULL	0	NULL	symptoms of diagnostic value	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that Cyps might play a role , probably as mediators in the pathophysiology of sepsis or as symptoms of diagnostic value .
	manualset3
106002	1	401773	13	NULL	NULL	0	NULL	increase in P	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that a significant increase in P triggers an LH surge and a single dose of Gesterol decreases E2/P ratio in the luteal phase of women after ovarian stimulation .
	manualset3
106004	2	401773	13	NULL	NULL	0	NULL	 LH surge	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that a significant increase in P triggers an LH surge and a single dose of Gesterol decreases E2/P ratio in the luteal phase of women after ovarian stimulation .
	manualset3
106007	3	401773	13	NULL	NULL	0	NULL	single dose of Gesterol	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that a significant increase in P triggers an LH surge and a single dose of Gesterol decreases E2/P ratio in the luteal phase of women after ovarian stimulation .
	manualset3
106009	4	401773	13	NULL	NULL	0	NULL	E2/P ratio	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that a significant increase in P triggers an LH surge and a single dose of Gesterol decreases E2/P ratio in the luteal phase of women after ovarian stimulation .
	manualset3
106011	5	401773	13	NULL	NULL	NULL	NULL	luteal phase	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is concluded that a significant increase in P triggers an LH surge and a single dose of Gesterol decreases E2/P ratio in the luteal phase of women after ovarian stimulation .
	manualset3
106013	6	401773	13	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that a significant increase in P triggers an LH surge and a single dose of Gesterol decreases E2/P ratio in the luteal phase of women after ovarian stimulation .
	manualset3
106014	7	401773	13	NULL	NULL	0	NULL	 ovarian stimulation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that a significant increase in P triggers an LH surge and a single dose of Gesterol decreases E2/P ratio in the luteal phase of women after ovarian stimulation .
	manualset3
106020	1	401774	13	NULL	NULL	0	NULL	adenosine agonists	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that adenosine and adenosine receptor agonists modulate glutamate release by activating inhibitory A1 and excitatory A2A receptors present on glutamatergic terminals of the rat cerebral cortex .
	manualset3
106021	2	401774	13	NULL	NULL	0	NULL	adenosine receptor agonists	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that adenosine and adenosine receptor agonists modulate glutamate release by activating inhibitory A1 and excitatory A2A receptors present on glutamatergic terminals of the rat cerebral cortex .
	manualset3
106022	3	401774	13	NULL	NULL	0	NULL	glutamate release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that adenosine and adenosine receptor agonists modulate glutamate release by activating inhibitory A1 and excitatory A2A receptors present on glutamatergic terminals of the rat cerebral cortex .
	manualset3
106026	4	401774	13	NULL	NULL	0	NULL	inhibitory A1 receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that adenosine and adenosine receptor agonists modulate glutamate release by activating inhibitory A1 and excitatory A2A receptors present on glutamatergic terminals of the rat cerebral cortex .
	manualset3
106027	5	401774	13	NULL	NULL	0	NULL	excitatory A2A receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that adenosine and adenosine receptor agonists modulate glutamate release by activating inhibitory A1 and excitatory A2A receptors present on glutamatergic terminals of the rat cerebral cortex .
	manualset3
106028	6	401774	13	NULL	NULL	0	NULL	glutamatergic terminals	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that adenosine and adenosine receptor agonists modulate glutamate release by activating inhibitory A1 and excitatory A2A receptors present on glutamatergic terminals of the rat cerebral cortex .
	manualset3
106030	7	401774	13	NULL	NULL	0	NULL	rat cerebral cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that adenosine and adenosine receptor agonists modulate glutamate release by activating inhibitory A1 and excitatory A2A receptors present on glutamatergic terminals of the rat cerebral cortex .
	manualset3
106032	1	401775	13	NULL	NULL	0	NULL	6 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	6 cases of lobar emphysema are reported .
	manualset3
106033	2	401775	13	NULL	NULL	0	NULL	lobar emphysema	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	6 cases of lobar emphysema are reported .
	manualset3
106037	1	401776	13	NULL	NULL	0	NULL	adrenergic mechanisms 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that adrenergic mechanisms contribute to the glucose-induced rise in splanchnic blood flow and thereby probably to the time course for intestinal absorption of nutrients .
	manualset3
106041	2	401776	13	NULL	NULL	0	NULL	glucose-induced rise 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that adrenergic mechanisms contribute to the glucose-induced rise in splanchnic blood flow and thereby probably to the time course for intestinal absorption of nutrients .
	manualset3
106042	3	401776	13	NULL	NULL	0	NULL	splanchnic blood flow	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that adrenergic mechanisms contribute to the glucose-induced rise in splanchnic blood flow and thereby probably to the time course for intestinal absorption of nutrients .
	manualset3
106043	4	401776	13	NULL	NULL	0	NULL	time course	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that adrenergic mechanisms contribute to the glucose-induced rise in splanchnic blood flow and thereby probably to the time course for intestinal absorption of nutrients .
	manualset3
106044	5	401776	13	NULL	NULL	0	NULL	intestinal absorption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that adrenergic mechanisms contribute to the glucose-induced rise in splanchnic blood flow and thereby probably to the time course for intestinal absorption of nutrients .
	manualset3
106045	6	401776	13	NULL	NULL	0	NULL	nutrients 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that adrenergic mechanisms contribute to the glucose-induced rise in splanchnic blood flow and thereby probably to the time course for intestinal absorption of nutrients .
	manualset3
106049	1	401777	13	NULL	NULL	0	NULL	assessment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that all assessment and prediction of suicide risk ultimately depends on the skill of the clinician .
	manualset3
106051	2	401777	13	NULL	NULL	0	NULL	prediction	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that all assessment and prediction of suicide risk ultimately depends on the skill of the clinician .
	manualset3
106052	3	401777	13	NULL	NULL	0	NULL	suicide risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that all assessment and prediction of suicide risk ultimately depends on the skill of the clinician .
	manualset3
106053	4	401777	13	NULL	NULL	NULL	NULL	skill	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is concluded that all assessment and prediction of suicide risk ultimately depends on the skill of the clinician .
	manualset3
106054	5	401777	13	NULL	NULL	0	NULL	clinician	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that all assessment and prediction of suicide risk ultimately depends on the skill of the clinician .
	manualset3
106081	1	401778	13	NULL	NULL	0	NULL	apomorphine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that apomorphine is a potent hydroxyl radical scavenger in vivo , especially for the dopamine formation .
	manualset3
106082	2	401778	13	NULL	NULL	0	NULL	 hydroxyl radical scavenger	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that apomorphine is a potent hydroxyl radical scavenger in vivo , especially for the dopamine formation .
	manualset3
106083	3	401778	13	NULL	NULL	0	NULL	dopamine formation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that apomorphine is a potent hydroxyl radical scavenger in vivo , especially for the dopamine formation .
	manualset3
106084	1	401779	13	NULL	NULL	0	NULL	level of accuracy	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that at the currently achievable level of accuracy , collective intramolecular motions are not essential for the interpretation of B-factors .
	manualset3
106085	2	401779	13	NULL	NULL	0	NULL	intramolecular motions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that at the currently achievable level of accuracy , collective intramolecular motions are not essential for the interpretation of B-factors .
	manualset3
106086	3	401779	13	NULL	NULL	0	NULL	 interpretation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that at the currently achievable level of accuracy , collective intramolecular motions are not essential for the interpretation of B-factors .
	manualset3
106087	4	401779	13	NULL	NULL	0	NULL	B-factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that at the currently achievable level of accuracy , collective intramolecular motions are not essential for the interpretation of B-factors .
	manualset3
106088	1	401780	13	NULL	NULL	0	NULL	deficiency of GSH	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that deficiency of GSH causes a marked increase in membrane permeability and such lenses are susceptible to oxidative damage resulting in inactivation of the Na + / K + pump , thus leading to ionic changes and cataract development .
	manualset3
106089	2	401780	13	NULL	NULL	0	NULL	increase in membrane permeability 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that deficiency of GSH causes a marked increase in membrane permeability and such lenses are susceptible to oxidative damage resulting in inactivation of the Na + / K + pump , thus leading to ionic changes and cataract development .
	manualset3
106090	3	401780	13	NULL	NULL	0	NULL	lenses  	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that deficiency of GSH causes a marked increase in membrane permeability and such lenses are susceptible to oxidative damage resulting in inactivation of the Na + / K + pump , thus leading to ionic changes and cataract development .
	manualset3
106091	4	401780	13	NULL	NULL	0	NULL	oxidative damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that deficiency of GSH causes a marked increase in membrane permeability and such lenses are susceptible to oxidative damage resulting in inactivation of the Na + / K + pump , thus leading to ionic changes and cataract development .
	manualset3
106092	5	401780	13	NULL	NULL	0	NULL	inactivation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that deficiency of GSH causes a marked increase in membrane permeability and such lenses are susceptible to oxidative damage resulting in inactivation of the Na + / K + pump , thus leading to ionic changes and cataract development .
	manualset3
106093	6	401780	13	NULL	NULL	0	NULL	 Na + / K + pump	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that deficiency of GSH causes a marked increase in membrane permeability and such lenses are susceptible to oxidative damage resulting in inactivation of the Na + / K + pump , thus leading to ionic changes and cataract development .
	manualset3
106094	7	401780	13	NULL	NULL	0	NULL	ionic changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that deficiency of GSH causes a marked increase in membrane permeability and such lenses are susceptible to oxidative damage resulting in inactivation of the Na + / K + pump , thus leading to ionic changes and cataract development .
	manualset3
106095	8	401780	13	NULL	NULL	0	NULL	cataract development	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that deficiency of GSH causes a marked increase in membrane permeability and such lenses are susceptible to oxidative damage resulting in inactivation of the Na + / K + pump , thus leading to ionic changes and cataract development .
	manualset3
106096	1	401781	13	NULL	NULL	0	NULL	dichloroacetate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that dichloroacetate may improve the metabolism of acetylcholine in activated cholinergic terminals by increasing the production of acetyl-CoA in mitochondria and increasing its provision through the mitochondrial membrane to synaptoplasm by the transport system , independent of the ATP-citrate lyase pathway .
	manualset3
106097	2	401781	13	NULL	NULL	0	NULL	metabolism of acetylcholine	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that dichloroacetate may improve the metabolism of acetylcholine in activated cholinergic terminals by increasing the production of acetyl-CoA in mitochondria and increasing its provision through the mitochondrial membrane to synaptoplasm by the transport system , independent of the ATP-citrate lyase pathway .
	manualset3
106100	3	401781	13	NULL	NULL	0	NULL	cholinergic terminals	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that dichloroacetate may improve the metabolism of acetylcholine in activated cholinergic terminals by increasing the production of acetyl-CoA in mitochondria and increasing its provision through the mitochondrial membrane to synaptoplasm by the transport system , independent of the ATP-citrate lyase pathway .
	manualset3
106102	4	401781	13	NULL	NULL	0	NULL	production of acetyl-CoA	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that dichloroacetate may improve the metabolism of acetylcholine in activated cholinergic terminals by increasing the production of acetyl-CoA in mitochondria and increasing its provision through the mitochondrial membrane to synaptoplasm by the transport system , independent of the ATP-citrate lyase pathway .
	manualset3
106103	5	401781	13	NULL	NULL	0	NULL	mitochondria 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that dichloroacetate may improve the metabolism of acetylcholine in activated cholinergic terminals by increasing the production of acetyl-CoA in mitochondria and increasing its provision through the mitochondrial membrane to synaptoplasm by the transport system , independent of the ATP-citrate lyase pathway .
	manualset3
106104	6	401781	13	NULL	NULL	0	NULL	 provision	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that dichloroacetate may improve the metabolism of acetylcholine in activated cholinergic terminals by increasing the production of acetyl-CoA in mitochondria and increasing its provision through the mitochondrial membrane to synaptoplasm by the transport system , independent of the ATP-citrate lyase pathway .
	manualset3
106105	7	401781	13	NULL	NULL	0	NULL	mitochondrial membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that dichloroacetate may improve the metabolism of acetylcholine in activated cholinergic terminals by increasing the production of acetyl-CoA in mitochondria and increasing its provision through the mitochondrial membrane to synaptoplasm by the transport system , independent of the ATP-citrate lyase pathway .
	manualset3
106107	8	401781	13	NULL	NULL	0	NULL	synaptoplasm	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that dichloroacetate may improve the metabolism of acetylcholine in activated cholinergic terminals by increasing the production of acetyl-CoA in mitochondria and increasing its provision through the mitochondrial membrane to synaptoplasm by the transport system , independent of the ATP-citrate lyase pathway .
	manualset3
106109	9	401781	13	NULL	NULL	0	NULL	transport system	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that dichloroacetate may improve the metabolism of acetylcholine in activated cholinergic terminals by increasing the production of acetyl-CoA in mitochondria and increasing its provision through the mitochondrial membrane to synaptoplasm by the transport system , independent of the ATP-citrate lyase pathway .
	manualset3
106110	10	401781	13	NULL	NULL	0	NULL	ATP-citrate lyase pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that dichloroacetate may improve the metabolism of acetylcholine in activated cholinergic terminals by increasing the production of acetyl-CoA in mitochondria and increasing its provision through the mitochondrial membrane to synaptoplasm by the transport system , independent of the ATP-citrate lyase pathway .
	manualset3
106111	1	401782	13	NULL	NULL	0	NULL	 inclusion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that dietary inclusion of SFO or SBO at 30 g/kg may alleviate the adverse effects of 0.3 microg/g of AF B1 in commercial broiler chickens .
	manualset3
106112	2	401782	13	NULL	NULL	0	NULL	SFO	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that dietary inclusion of SFO or SBO at 30 g/kg may alleviate the adverse effects of 0.3 microg/g of AF B1 in commercial broiler chickens .
	manualset3
106113	3	401782	13	NULL	NULL	0	NULL	SBO	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that dietary inclusion of SFO or SBO at 30 g/kg may alleviate the adverse effects of 0.3 microg/g of AF B1 in commercial broiler chickens .
	manualset3
106114	4	401782	13	NULL	NULL	0	NULL	30 g/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that dietary inclusion of SFO or SBO at 30 g/kg may alleviate the adverse effects of 0.3 microg/g of AF B1 in commercial broiler chickens .
	manualset3
106116	5	401782	13	NULL	NULL	0	NULL	 adverse effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that dietary inclusion of SFO or SBO at 30 g/kg may alleviate the adverse effects of 0.3 microg/g of AF B1 in commercial broiler chickens .
	manualset3
106118	6	401782	13	NULL	NULL	0	NULL	0.3 microg/g 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that dietary inclusion of SFO or SBO at 30 g/kg may alleviate the adverse effects of 0.3 microg/g of AF B1 in commercial broiler chickens .
	manualset3
106123	7	401782	13	NULL	NULL	0	NULL	AF B1 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that dietary inclusion of SFO or SBO at 30 g/kg may alleviate the adverse effects of 0.3 microg/g of AF B1 in commercial broiler chickens .
	manualset3
106124	8	401782	13	NULL	NULL	0	NULL	broiler chickens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that dietary inclusion of SFO or SBO at 30 g/kg may alleviate the adverse effects of 0.3 microg/g of AF B1 in commercial broiler chickens .
	manualset3
106134	1	401783	13	NULL	NULL	0	NULL	dietary selenium	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that dietary selenium inhibits pulmonary cell proliferation in both control and cigarette smoke-exposed mice , indicating that selenium is inhibiting cell proliferation independently of smoke exposure , and that this inhibition may be related to selenium concentration and GPx activity in the lung .
	manualset3
106135	2	401783	13	NULL	NULL	0	NULL	pulmonary cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that dietary selenium inhibits pulmonary cell proliferation in both control and cigarette smoke-exposed mice , indicating that selenium is inhibiting cell proliferation independently of smoke exposure , and that this inhibition may be related to selenium concentration and GPx activity in the lung .
	manualset3
106137	3	401783	13	NULL	NULL	0	NULL	control mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that dietary selenium inhibits pulmonary cell proliferation in both control and cigarette smoke-exposed mice , indicating that selenium is inhibiting cell proliferation independently of smoke exposure , and that this inhibition may be related to selenium concentration and GPx activity in the lung .
	manualset3
106139	4	401783	13	NULL	NULL	0	NULL	cigarette smoke-exposed mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that dietary selenium inhibits pulmonary cell proliferation in both control and cigarette smoke-exposed mice , indicating that selenium is inhibiting cell proliferation independently of smoke exposure , and that this inhibition may be related to selenium concentration and GPx activity in the lung .
	manualset3
106141	5	401783	13	NULL	NULL	0	NULL	selenium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that dietary selenium inhibits pulmonary cell proliferation in both control and cigarette smoke-exposed mice , indicating that selenium is inhibiting cell proliferation independently of smoke exposure , and that this inhibition may be related to selenium concentration and GPx activity in the lung .
	manualset3
106142	6	401783	13	NULL	NULL	0	NULL	cell proliferation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that dietary selenium inhibits pulmonary cell proliferation in both control and cigarette smoke-exposed mice , indicating that selenium is inhibiting cell proliferation independently of smoke exposure , and that this inhibition may be related to selenium concentration and GPx activity in the lung .
	manualset3
106144	7	401783	13	NULL	NULL	0	NULL	smoke exposure 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that dietary selenium inhibits pulmonary cell proliferation in both control and cigarette smoke-exposed mice , indicating that selenium is inhibiting cell proliferation independently of smoke exposure , and that this inhibition may be related to selenium concentration and GPx activity in the lung .
	manualset3
106145	8	401783	13	NULL	NULL	0	NULL	inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that dietary selenium inhibits pulmonary cell proliferation in both control and cigarette smoke-exposed mice , indicating that selenium is inhibiting cell proliferation independently of smoke exposure , and that this inhibition may be related to selenium concentration and GPx activity in the lung .
	manualset3
106146	9	401783	13	NULL	NULL	0	NULL	selenium concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that dietary selenium inhibits pulmonary cell proliferation in both control and cigarette smoke-exposed mice , indicating that selenium is inhibiting cell proliferation independently of smoke exposure , and that this inhibition may be related to selenium concentration and GPx activity in the lung .
	manualset3
106147	10	401783	13	NULL	NULL	0	NULL	GPx activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that dietary selenium inhibits pulmonary cell proliferation in both control and cigarette smoke-exposed mice , indicating that selenium is inhibiting cell proliferation independently of smoke exposure , and that this inhibition may be related to selenium concentration and GPx activity in the lung .
	manualset3
106148	11	401783	13	NULL	NULL	0	NULL	lung	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that dietary selenium inhibits pulmonary cell proliferation in both control and cigarette smoke-exposed mice , indicating that selenium is inhibiting cell proliferation independently of smoke exposure , and that this inhibition may be related to selenium concentration and GPx activity in the lung .
	manualset3
106150	1	401784	13	NULL	NULL	0	NULL	droperidol 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that droperidol reduces the renal vasodilatation induced by dopamine in anaesthetized dogs .
	manualset3
106153	2	401784	13	NULL	NULL	0	NULL	renal vasodilatation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that droperidol reduces the renal vasodilatation induced by dopamine in anaesthetized dogs .
	manualset3
106154	3	401784	13	NULL	NULL	0	NULL	dopamine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that droperidol reduces the renal vasodilatation induced by dopamine in anaesthetized dogs .
	manualset3
106156	4	401784	13	NULL	NULL	0	NULL	anaesthetized dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that droperidol reduces the renal vasodilatation induced by dopamine in anaesthetized dogs .
	manualset3
106157	1	401785	13	NULL	NULL	0	NULL	dynamic changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that due to marked dynamic changes in unmeasured ionic composition of neonatal urine UAG is not a valuable index of urinary ammonium excretion in newborn infants during the first weeks of life .
	manualset3
106158	2	401785	13	NULL	NULL	0	NULL	ionic composition	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that due to marked dynamic changes in unmeasured ionic composition of neonatal urine UAG is not a valuable index of urinary ammonium excretion in newborn infants during the first weeks of life .
	manualset3
106159	3	401785	13	NULL	NULL	0	NULL	neonatal urine UAG	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that due to marked dynamic changes in unmeasured ionic composition of neonatal urine UAG is not a valuable index of urinary ammonium excretion in newborn infants during the first weeks of life .
	manualset3
106160	4	401785	13	NULL	NULL	0	NULL	valuable index 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that due to marked dynamic changes in unmeasured ionic composition of neonatal urine UAG is not a valuable index of urinary ammonium excretion in newborn infants during the first weeks of life .
	manualset3
106161	5	401785	13	NULL	NULL	0	NULL	urinary ammonium excretion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that due to marked dynamic changes in unmeasured ionic composition of neonatal urine UAG is not a valuable index of urinary ammonium excretion in newborn infants during the first weeks of life .
	manualset3
106162	6	401785	13	NULL	NULL	0	NULL	newborn infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that due to marked dynamic changes in unmeasured ionic composition of neonatal urine UAG is not a valuable index of urinary ammonium excretion in newborn infants during the first weeks of life .
	manualset3
106164	7	401785	13	NULL	NULL	0	NULL	first weeks of life	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that due to marked dynamic changes in unmeasured ionic composition of neonatal urine UAG is not a valuable index of urinary ammonium excretion in newborn infants during the first weeks of life .
	manualset3
106183	1	401786	13	NULL	NULL	0	NULL	6 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	6 eyes had undergone ICCE and one eye had been secondarily implanted .
	manualset3
106184	2	401786	13	NULL	NULL	0	NULL	eyes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	6 eyes had undergone ICCE and one eye had been secondarily implanted .
	manualset3
106185	3	401786	13	NULL	NULL	0	NULL	ICCE	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	6 eyes had undergone ICCE and one eye had been secondarily implanted .
	manualset3
106186	4	401786	13	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	6 eyes had undergone ICCE and one eye had been secondarily implanted .
	manualset3
106187	5	401786	13	NULL	NULL	0	NULL	eye 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	6 eyes had undergone ICCE and one eye had been secondarily implanted .
	manualset3
106188	1	401787	13	NULL	NULL	0	NULL	hyaluronidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that hyaluronidase increases the rate of absorption of succinylcholine chloride .
	manualset3
106189	2	401787	13	NULL	NULL	0	NULL	rate of absorption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that hyaluronidase increases the rate of absorption of succinylcholine chloride .
	manualset3
106190	3	401787	13	NULL	NULL	0	NULL	succinylcholine chloride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that hyaluronidase increases the rate of absorption of succinylcholine chloride .
	manualset3
106191	1	401788	13	NULL	NULL	0	NULL	level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that increased level of adiponectin has no significant antiaggregation effect on platelets from individuals without hypoadiponectinemia .
	manualset3
106192	2	401788	13	NULL	NULL	0	NULL	adiponectin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that increased level of adiponectin has no significant antiaggregation effect on platelets from individuals without hypoadiponectinemia .
	manualset3
106193	3	401788	13	NULL	NULL	0	NULL	 antiaggregation effect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that increased level of adiponectin has no significant antiaggregation effect on platelets from individuals without hypoadiponectinemia .
	manualset3
106194	4	401788	13	NULL	NULL	NULL	NULL	platelets	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is concluded that increased level of adiponectin has no significant antiaggregation effect on platelets from individuals without hypoadiponectinemia .
	manualset3
106195	5	401788	13	NULL	NULL	0	NULL	individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that increased level of adiponectin has no significant antiaggregation effect on platelets from individuals without hypoadiponectinemia .
	manualset3
106196	6	401788	13	NULL	NULL	0	NULL	hypoadiponectinemia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that increased level of adiponectin has no significant antiaggregation effect on platelets from individuals without hypoadiponectinemia .
	manualset3
106197	1	401789	13	NULL	NULL	0	NULL	infection per se	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that infection per se is not the cause of the elevated SRL .
	manualset3
106198	2	401789	13	NULL	NULL	0	NULL	cause 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that infection per se is not the cause of the elevated SRL .
	manualset3
106199	3	401789	13	NULL	NULL	0	NULL	SRL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that infection per se is not the cause of the elevated SRL .
	manualset3
106200	1	401790	13	NULL	NULL	0	NULL	 neck vein catheterisation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that neck vein catheterisation and parathyroid hormone assay can correctly localize parathyroid tumors in most cases of primary hyperparathyroidism , but it is suggested that its use be restricted to selected cases such as those subjects with previous negative neck exploration or patients for whom prolonged or repeated surgery may be a particular hazard .
	manualset3
106201	2	401790	13	NULL	NULL	0	NULL	parathyroid hormone assay 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that neck vein catheterisation and parathyroid hormone assay can correctly localize parathyroid tumors in most cases of primary hyperparathyroidism , but it is suggested that its use be restricted to selected cases such as those subjects with previous negative neck exploration or patients for whom prolonged or repeated surgery may be a particular hazard .
	manualset3
106202	3	401790	13	NULL	NULL	0	NULL	parathyroid tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that neck vein catheterisation and parathyroid hormone assay can correctly localize parathyroid tumors in most cases of primary hyperparathyroidism , but it is suggested that its use be restricted to selected cases such as those subjects with previous negative neck exploration or patients for whom prolonged or repeated surgery may be a particular hazard .
	manualset3
106203	4	401790	13	NULL	NULL	NULL	NULL	cases	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is concluded that neck vein catheterisation and parathyroid hormone assay can correctly localize parathyroid tumors in most cases of primary hyperparathyroidism , but it is suggested that its use be restricted to selected cases such as those subjects with previous negative neck exploration or patients for whom prolonged or repeated surgery may be a particular hazard .
	manualset3
106204	5	401790	13	NULL	NULL	0	NULL	primary hyperparathyroidism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that neck vein catheterisation and parathyroid hormone assay can correctly localize parathyroid tumors in most cases of primary hyperparathyroidism , but it is suggested that its use be restricted to selected cases such as those subjects with previous negative neck exploration or patients for whom prolonged or repeated surgery may be a particular hazard .
	manualset3
106205	6	401790	13	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that neck vein catheterisation and parathyroid hormone assay can correctly localize parathyroid tumors in most cases of primary hyperparathyroidism , but it is suggested that its use be restricted to selected cases such as those subjects with previous negative neck exploration or patients for whom prolonged or repeated surgery may be a particular hazard .
	manualset3
106206	7	401790	13	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that neck vein catheterisation and parathyroid hormone assay can correctly localize parathyroid tumors in most cases of primary hyperparathyroidism , but it is suggested that its use be restricted to selected cases such as those subjects with previous negative neck exploration or patients for whom prolonged or repeated surgery may be a particular hazard .
	manualset3
106207	8	401790	13	NULL	NULL	0	NULL	subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that neck vein catheterisation and parathyroid hormone assay can correctly localize parathyroid tumors in most cases of primary hyperparathyroidism , but it is suggested that its use be restricted to selected cases such as those subjects with previous negative neck exploration or patients for whom prolonged or repeated surgery may be a particular hazard .
	manualset3
106209	9	401790	13	NULL	NULL	0	NULL	negative neck exploration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that neck vein catheterisation and parathyroid hormone assay can correctly localize parathyroid tumors in most cases of primary hyperparathyroidism , but it is suggested that its use be restricted to selected cases such as those subjects with previous negative neck exploration or patients for whom prolonged or repeated surgery may be a particular hazard .
	manualset3
106210	10	401790	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that neck vein catheterisation and parathyroid hormone assay can correctly localize parathyroid tumors in most cases of primary hyperparathyroidism , but it is suggested that its use be restricted to selected cases such as those subjects with previous negative neck exploration or patients for whom prolonged or repeated surgery may be a particular hazard .
	manualset3
106212	11	401790	13	NULL	NULL	0	NULL	prolonged surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that neck vein catheterisation and parathyroid hormone assay can correctly localize parathyroid tumors in most cases of primary hyperparathyroidism , but it is suggested that its use be restricted to selected cases such as those subjects with previous negative neck exploration or patients for whom prolonged or repeated surgery may be a particular hazard .
	manualset3
106213	12	401790	13	NULL	NULL	0	NULL	repeated surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that neck vein catheterisation and parathyroid hormone assay can correctly localize parathyroid tumors in most cases of primary hyperparathyroidism , but it is suggested that its use be restricted to selected cases such as those subjects with previous negative neck exploration or patients for whom prolonged or repeated surgery may be a particular hazard .
	manualset3
106214	13	401790	13	NULL	NULL	0	NULL	particular hazard	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that neck vein catheterisation and parathyroid hormone assay can correctly localize parathyroid tumors in most cases of primary hyperparathyroidism , but it is suggested that its use be restricted to selected cases such as those subjects with previous negative neck exploration or patients for whom prolonged or repeated surgery may be a particular hazard .
	manualset3
106216	1	401791	13	NULL	NULL	0	NULL	reactive astrocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that reactive astrocytes from adult host central nervous system migrate into peripheral ganglionic transplants , where they differentiate and establish organized arrangements with the ganglionic elements .
	manualset3
106217	2	401791	13	NULL	NULL	NULL	NULL	adult host	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is concluded that reactive astrocytes from adult host central nervous system migrate into peripheral ganglionic transplants , where they differentiate and establish organized arrangements with the ganglionic elements .
	manualset3
106218	3	401791	13	NULL	NULL	0	NULL	central nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that reactive astrocytes from adult host central nervous system migrate into peripheral ganglionic transplants , where they differentiate and establish organized arrangements with the ganglionic elements .
	manualset3
106219	4	401791	13	NULL	NULL	0	NULL	peripheral ganglionic transplants	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that reactive astrocytes from adult host central nervous system migrate into peripheral ganglionic transplants , where they differentiate and establish organized arrangements with the ganglionic elements .
	manualset3
106221	5	401791	13	NULL	NULL	0	NULL	arrangements 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that reactive astrocytes from adult host central nervous system migrate into peripheral ganglionic transplants , where they differentiate and establish organized arrangements with the ganglionic elements .
	manualset3
106222	6	401791	13	NULL	NULL	0	NULL	ganglionic elements	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that reactive astrocytes from adult host central nervous system migrate into peripheral ganglionic transplants , where they differentiate and establish organized arrangements with the ganglionic elements .
	manualset3
106229	1	401792	13	NULL	NULL	0	NULL	stimulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that stimulation of Ch uptake and ACh synthesis by nerve activity depends first , on the ACh release elicited by Ca + + influx after depolarization and second , on the activation of the Na , K-ATPase due to Na + entry .
	manualset3
106230	2	401792	13	NULL	NULL	0	NULL	Ch uptake	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that stimulation of Ch uptake and ACh synthesis by nerve activity depends first , on the ACh release elicited by Ca + + influx after depolarization and second , on the activation of the Na , K-ATPase due to Na + entry .
	manualset3
106231	3	401792	13	NULL	NULL	0	NULL	ACh synthesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that stimulation of Ch uptake and ACh synthesis by nerve activity depends first , on the ACh release elicited by Ca + + influx after depolarization and second , on the activation of the Na , K-ATPase due to Na + entry .
	manualset3
106232	4	401792	13	NULL	NULL	0	NULL	nerve activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that stimulation of Ch uptake and ACh synthesis by nerve activity depends first , on the ACh release elicited by Ca + + influx after depolarization and second , on the activation of the Na , K-ATPase due to Na + entry .
	manualset3
106233	5	401792	13	NULL	NULL	0	NULL	ACh release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that stimulation of Ch uptake and ACh synthesis by nerve activity depends first , on the ACh release elicited by Ca + + influx after depolarization and second , on the activation of the Na , K-ATPase due to Na + entry .
	manualset3
106234	6	401792	13	NULL	NULL	0	NULL	Ca + + influx 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that stimulation of Ch uptake and ACh synthesis by nerve activity depends first , on the ACh release elicited by Ca + + influx after depolarization and second , on the activation of the Na , K-ATPase due to Na + entry .
	manualset3
106235	7	401792	13	NULL	NULL	0	NULL	depolarization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that stimulation of Ch uptake and ACh synthesis by nerve activity depends first , on the ACh release elicited by Ca + + influx after depolarization and second , on the activation of the Na , K-ATPase due to Na + entry .
	manualset3
106236	8	401792	13	NULL	NULL	0	NULL	 activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that stimulation of Ch uptake and ACh synthesis by nerve activity depends first , on the ACh release elicited by Ca + + influx after depolarization and second , on the activation of the Na , K-ATPase due to Na + entry .
	manualset3
106237	9	401792	13	NULL	NULL	0	NULL	Na , K-ATPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that stimulation of Ch uptake and ACh synthesis by nerve activity depends first , on the ACh release elicited by Ca + + influx after depolarization and second , on the activation of the Na , K-ATPase due to Na + entry .
	manualset3
106238	10	401792	13	NULL	NULL	0	NULL	Na + entry 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that stimulation of Ch uptake and ACh synthesis by nerve activity depends first , on the ACh release elicited by Ca + + influx after depolarization and second , on the activation of the Na , K-ATPase due to Na + entry .
	manualset3
106239	1	401793	13	NULL	NULL	0	NULL	GAFF/TIP3P combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the GAFF/TIP3P combination can be utilized for aqueous membrane bilayer simulations , as it provides acceptable accuracy for biomolecular modeling .
	manualset3
106240	2	401793	13	NULL	NULL	0	NULL	aqueous membrane bilayer simulations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the GAFF/TIP3P combination can be utilized for aqueous membrane bilayer simulations , as it provides acceptable accuracy for biomolecular modeling .
	manualset3
106241	3	401793	13	NULL	NULL	0	NULL	accuracy	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the GAFF/TIP3P combination can be utilized for aqueous membrane bilayer simulations , as it provides acceptable accuracy for biomolecular modeling .
	manualset3
106242	4	401793	13	NULL	NULL	0	NULL	biomolecular modeling 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the GAFF/TIP3P combination can be utilized for aqueous membrane bilayer simulations , as it provides acceptable accuracy for biomolecular modeling .
	manualset3
106243	1	401794	13	NULL	NULL	0	NULL	absorption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the absorption of deramciclane , and possibly other acid-labile drugs , can not be predicted by use of the dog model .
	manualset3
106244	2	401794	13	NULL	NULL	0	NULL	deramciclane	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the absorption of deramciclane , and possibly other acid-labile drugs , can not be predicted by use of the dog model .
	manualset3
106245	3	401794	13	NULL	NULL	0	NULL	acid-labile drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the absorption of deramciclane , and possibly other acid-labile drugs , can not be predicted by use of the dog model .
	manualset3
106246	4	401794	13	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the absorption of deramciclane , and possibly other acid-labile drugs , can not be predicted by use of the dog model .
	manualset3
106247	5	401794	13	NULL	NULL	0	NULL	dog model 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the absorption of deramciclane , and possibly other acid-labile drugs , can not be predicted by use of the dog model .
	manualset3
106248	1	401795	13	NULL	NULL	NULL	NULL	biological characteristics 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is concluded that the biological characteristics of osteoblasts from bone marrow of MDS patients are generally not different from those of osteoblasts from normal bone marrow .
	manualset3
106249	2	401795	13	NULL	NULL	0	NULL	osteoblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the biological characteristics of osteoblasts from bone marrow of MDS patients are generally not different from those of osteoblasts from normal bone marrow .
	manualset3
106250	3	401795	13	NULL	NULL	0	NULL	bone marrow	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the biological characteristics of osteoblasts from bone marrow of MDS patients are generally not different from those of osteoblasts from normal bone marrow .
	manualset3
106251	4	401795	13	NULL	NULL	0	NULL	MDS patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the biological characteristics of osteoblasts from bone marrow of MDS patients are generally not different from those of osteoblasts from normal bone marrow .
	manualset3
106252	5	401795	13	NULL	NULL	0	NULL	osteoblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the biological characteristics of osteoblasts from bone marrow of MDS patients are generally not different from those of osteoblasts from normal bone marrow .
	manualset3
106253	6	401795	13	NULL	NULL	0	NULL	normal bone marrow	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the biological characteristics of osteoblasts from bone marrow of MDS patients are generally not different from those of osteoblasts from normal bone marrow .
	manualset3
106254	1	401796	13	NULL	NULL	0	NULL	60-90 days 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	60-90 days after infection , worm-cysts can not only be detected in the lungs , but also in the liver , mediastinum and abdominal wall , with mature or premature worms and eggs .
	manualset3
106255	2	401796	13	NULL	NULL	0	NULL	 infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	60-90 days after infection , worm-cysts can not only be detected in the lungs , but also in the liver , mediastinum and abdominal wall , with mature or premature worms and eggs .
	manualset3
106256	3	401796	13	NULL	NULL	0	NULL	worm-cysts	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	60-90 days after infection , worm-cysts can not only be detected in the lungs , but also in the liver , mediastinum and abdominal wall , with mature or premature worms and eggs .
	manualset3
106257	4	401796	13	NULL	NULL	0	NULL	 lungs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	60-90 days after infection , worm-cysts can not only be detected in the lungs , but also in the liver , mediastinum and abdominal wall , with mature or premature worms and eggs .
	manualset3
106258	5	401796	13	NULL	NULL	0	NULL	 liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	60-90 days after infection , worm-cysts can not only be detected in the lungs , but also in the liver , mediastinum and abdominal wall , with mature or premature worms and eggs .
	manualset3
106259	6	401796	13	NULL	NULL	0	NULL	mediastinum 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	60-90 days after infection , worm-cysts can not only be detected in the lungs , but also in the liver , mediastinum and abdominal wall , with mature or premature worms and eggs .
	manualset3
106260	7	401796	13	NULL	NULL	0	NULL	abdominal wall	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	60-90 days after infection , worm-cysts can not only be detected in the lungs , but also in the liver , mediastinum and abdominal wall , with mature or premature worms and eggs .
	manualset3
106261	8	401796	13	NULL	NULL	0	NULL	mature worms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	60-90 days after infection , worm-cysts can not only be detected in the lungs , but also in the liver , mediastinum and abdominal wall , with mature or premature worms and eggs .
	manualset3
106263	9	401796	13	NULL	NULL	0	NULL	 premature worms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	60-90 days after infection , worm-cysts can not only be detected in the lungs , but also in the liver , mediastinum and abdominal wall , with mature or premature worms and eggs .
	manualset3
106264	10	401796	13	NULL	NULL	0	NULL	eggs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	60-90 days after infection , worm-cysts can not only be detected in the lungs , but also in the liver , mediastinum and abdominal wall , with mature or premature worms and eggs .
	manualset3
106265	1	401797	13	NULL	NULL	0	NULL	deficit in IQ score	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the deficit in IQ score found at 3 and 5 years in children with severe hypothyroidism is still evident at the age of 10 years .
	manualset3
106266	2	401797	13	NULL	NULL	0	NULL	3 years	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the deficit in IQ score found at 3 and 5 years in children with severe hypothyroidism is still evident at the age of 10 years .
	manualset3
106267	3	401797	13	NULL	NULL	0	NULL	5 years	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the deficit in IQ score found at 3 and 5 years in children with severe hypothyroidism is still evident at the age of 10 years .
	manualset3
106268	4	401797	13	NULL	NULL	0	NULL	 children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the deficit in IQ score found at 3 and 5 years in children with severe hypothyroidism is still evident at the age of 10 years .
	manualset3
106269	5	401797	13	NULL	NULL	0	NULL	severe hypothyroidism 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the deficit in IQ score found at 3 and 5 years in children with severe hypothyroidism is still evident at the age of 10 years .
	manualset3
106270	6	401797	13	NULL	NULL	0	NULL	age of 10 years	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the deficit in IQ score found at 3 and 5 years in children with severe hypothyroidism is still evident at the age of 10 years .
	manualset3
106271	1	401798	13	NULL	NULL	0	NULL	pathways	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the pathways subserving lower-urinary-tract function are closely associated with the pathways subserving pinprick sensation , and that a lesion along the spinal axis can affect the bladder , sphincter , or both in a variety of ways , thus leading to the widely variable clinical findings associated with neurogenic lower urinary tract dysfunction .
	manualset3
106272	2	401798	13	NULL	NULL	0	NULL	lower-urinary-tract function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the pathways subserving lower-urinary-tract function are closely associated with the pathways subserving pinprick sensation , and that a lesion along the spinal axis can affect the bladder , sphincter , or both in a variety of ways , thus leading to the widely variable clinical findings associated with neurogenic lower urinary tract dysfunction .
	manualset3
106273	3	401798	13	NULL	NULL	0	NULL	pathways	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the pathways subserving lower-urinary-tract function are closely associated with the pathways subserving pinprick sensation , and that a lesion along the spinal axis can affect the bladder , sphincter , or both in a variety of ways , thus leading to the widely variable clinical findings associated with neurogenic lower urinary tract dysfunction .
	manualset3
106274	4	401798	13	NULL	NULL	0	NULL	pinprick sensation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the pathways subserving lower-urinary-tract function are closely associated with the pathways subserving pinprick sensation , and that a lesion along the spinal axis can affect the bladder , sphincter , or both in a variety of ways , thus leading to the widely variable clinical findings associated with neurogenic lower urinary tract dysfunction .
	manualset3
106275	5	401798	13	NULL	NULL	0	NULL	lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the pathways subserving lower-urinary-tract function are closely associated with the pathways subserving pinprick sensation , and that a lesion along the spinal axis can affect the bladder , sphincter , or both in a variety of ways , thus leading to the widely variable clinical findings associated with neurogenic lower urinary tract dysfunction .
	manualset3
106276	6	401798	13	NULL	NULL	0	NULL	spinal axis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the pathways subserving lower-urinary-tract function are closely associated with the pathways subserving pinprick sensation , and that a lesion along the spinal axis can affect the bladder , sphincter , or both in a variety of ways , thus leading to the widely variable clinical findings associated with neurogenic lower urinary tract dysfunction .
	manualset3
106277	7	401798	13	NULL	NULL	0	NULL	bladder	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the pathways subserving lower-urinary-tract function are closely associated with the pathways subserving pinprick sensation , and that a lesion along the spinal axis can affect the bladder , sphincter , or both in a variety of ways , thus leading to the widely variable clinical findings associated with neurogenic lower urinary tract dysfunction .
	manualset3
106278	8	401798	13	NULL	NULL	0	NULL	sphincter	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the pathways subserving lower-urinary-tract function are closely associated with the pathways subserving pinprick sensation , and that a lesion along the spinal axis can affect the bladder , sphincter , or both in a variety of ways , thus leading to the widely variable clinical findings associated with neurogenic lower urinary tract dysfunction .
	manualset3
106279	9	401798	13	NULL	NULL	0	NULL	variety of ways	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the pathways subserving lower-urinary-tract function are closely associated with the pathways subserving pinprick sensation , and that a lesion along the spinal axis can affect the bladder , sphincter , or both in a variety of ways , thus leading to the widely variable clinical findings associated with neurogenic lower urinary tract dysfunction .
	manualset3
106280	10	401798	13	NULL	NULL	0	NULL	clinical findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the pathways subserving lower-urinary-tract function are closely associated with the pathways subserving pinprick sensation , and that a lesion along the spinal axis can affect the bladder , sphincter , or both in a variety of ways , thus leading to the widely variable clinical findings associated with neurogenic lower urinary tract dysfunction .
	manualset3
106281	11	401798	13	NULL	NULL	0	NULL	neurogenic lower urinary tract dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the pathways subserving lower-urinary-tract function are closely associated with the pathways subserving pinprick sensation , and that a lesion along the spinal axis can affect the bladder , sphincter , or both in a variety of ways , thus leading to the widely variable clinical findings associated with neurogenic lower urinary tract dysfunction .
	manualset3
106282	1	401799	13	NULL	NULL	0	NULL	variations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the variations of the amide C = O stretching mode frequency can be used for quantitative characterization of the amide group conformational flexibility in the studied series of acetanilides .
	manualset3
106283	2	401799	13	NULL	NULL	NULL	NULL	amide C = O 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is concluded that the variations of the amide C = O stretching mode frequency can be used for quantitative characterization of the amide group conformational flexibility in the studied series of acetanilides .
	manualset3
106284	3	401799	13	NULL	NULL	0	NULL	frequency 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the variations of the amide C = O stretching mode frequency can be used for quantitative characterization of the amide group conformational flexibility in the studied series of acetanilides .
	manualset3
106285	4	401799	13	NULL	NULL	0	NULL	quantitative characterization	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the variations of the amide C = O stretching mode frequency can be used for quantitative characterization of the amide group conformational flexibility in the studied series of acetanilides .
	manualset3
106286	5	401799	13	NULL	NULL	0	NULL	amide group	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the variations of the amide C = O stretching mode frequency can be used for quantitative characterization of the amide group conformational flexibility in the studied series of acetanilides .
	manualset3
106287	6	401799	13	NULL	NULL	0	NULL	conformational flexibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the variations of the amide C = O stretching mode frequency can be used for quantitative characterization of the amide group conformational flexibility in the studied series of acetanilides .
	manualset3
106288	7	401799	13	NULL	NULL	0	NULL	series of acetanilides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the variations of the amide C = O stretching mode frequency can be used for quantitative characterization of the amide group conformational flexibility in the studied series of acetanilides .
	manualset3
106289	1	401800	13	NULL	NULL	0	NULL	therapeutic moderate hypothermia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that therapeutic moderate hypothermia is safe and has sustained favorable effects on acute derangements of cerebral physiology and metabolism caused by severe closed head injury .
	manualset3
106290	2	401800	13	NULL	NULL	0	NULL	favorable effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that therapeutic moderate hypothermia is safe and has sustained favorable effects on acute derangements of cerebral physiology and metabolism caused by severe closed head injury .
	manualset3
106291	3	401800	13	NULL	NULL	0	NULL	acute derangements 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that therapeutic moderate hypothermia is safe and has sustained favorable effects on acute derangements of cerebral physiology and metabolism caused by severe closed head injury .
	manualset3
106292	4	401800	13	NULL	NULL	0	NULL	cerebral physiology	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that therapeutic moderate hypothermia is safe and has sustained favorable effects on acute derangements of cerebral physiology and metabolism caused by severe closed head injury .
	manualset3
106293	5	401800	13	NULL	NULL	0	NULL	metabolism 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that therapeutic moderate hypothermia is safe and has sustained favorable effects on acute derangements of cerebral physiology and metabolism caused by severe closed head injury .
	manualset3
106294	6	401800	13	NULL	NULL	0	NULL	severe closed head injury 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that therapeutic moderate hypothermia is safe and has sustained favorable effects on acute derangements of cerebral physiology and metabolism caused by severe closed head injury .
	manualset3
106295	1	401801	13	NULL	NULL	0	NULL	tolbutamide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that tolbutamide has two opposing actions on islet beta-cell 86Rb efflux , and therefore PK : ( i ) a tendency to increase a calcium-sensitive PK by stimulating calcium entry into the cell and ( ii ) a decrease in PK that may be due to a direct effect on the calcium-sensitive PK itself .
	manualset3
106296	2	401801	13	NULL	NULL	0	NULL	actions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that tolbutamide has two opposing actions on islet beta-cell 86Rb efflux , and therefore PK : ( i ) a tendency to increase a calcium-sensitive PK by stimulating calcium entry into the cell and ( ii ) a decrease in PK that may be due to a direct effect on the calcium-sensitive PK itself .
	manualset3
106297	3	401801	13	NULL	NULL	0	NULL	islet beta-cell 86Rb efflux	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that tolbutamide has two opposing actions on islet beta-cell 86Rb efflux , and therefore PK : ( i ) a tendency to increase a calcium-sensitive PK by stimulating calcium entry into the cell and ( ii ) a decrease in PK that may be due to a direct effect on the calcium-sensitive PK itself .
	manualset3
106298	4	401801	13	NULL	NULL	0	NULL	 PK 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that tolbutamide has two opposing actions on islet beta-cell 86Rb efflux , and therefore PK : ( i ) a tendency to increase a calcium-sensitive PK by stimulating calcium entry into the cell and ( ii ) a decrease in PK that may be due to a direct effect on the calcium-sensitive PK itself .
	manualset3
106299	5	401801	13	NULL	NULL	0	NULL	tendency 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that tolbutamide has two opposing actions on islet beta-cell 86Rb efflux , and therefore PK : ( i ) a tendency to increase a calcium-sensitive PK by stimulating calcium entry into the cell and ( ii ) a decrease in PK that may be due to a direct effect on the calcium-sensitive PK itself .
	manualset3
106300	6	401801	13	NULL	NULL	0	NULL	calcium-sensitive PK	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that tolbutamide has two opposing actions on islet beta-cell 86Rb efflux , and therefore PK : ( i ) a tendency to increase a calcium-sensitive PK by stimulating calcium entry into the cell and ( ii ) a decrease in PK that may be due to a direct effect on the calcium-sensitive PK itself .
	manualset3
106301	7	401801	13	NULL	NULL	0	NULL	calcium entry	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that tolbutamide has two opposing actions on islet beta-cell 86Rb efflux , and therefore PK : ( i ) a tendency to increase a calcium-sensitive PK by stimulating calcium entry into the cell and ( ii ) a decrease in PK that may be due to a direct effect on the calcium-sensitive PK itself .
	manualset3
106302	8	401801	13	NULL	NULL	0	NULL	cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that tolbutamide has two opposing actions on islet beta-cell 86Rb efflux , and therefore PK : ( i ) a tendency to increase a calcium-sensitive PK by stimulating calcium entry into the cell and ( ii ) a decrease in PK that may be due to a direct effect on the calcium-sensitive PK itself .
	manualset3
106303	9	401801	13	NULL	NULL	0	NULL	decrease in PK	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that tolbutamide has two opposing actions on islet beta-cell 86Rb efflux , and therefore PK : ( i ) a tendency to increase a calcium-sensitive PK by stimulating calcium entry into the cell and ( ii ) a decrease in PK that may be due to a direct effect on the calcium-sensitive PK itself .
	manualset3
106304	10	401801	13	NULL	NULL	0	NULL	effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that tolbutamide has two opposing actions on islet beta-cell 86Rb efflux , and therefore PK : ( i ) a tendency to increase a calcium-sensitive PK by stimulating calcium entry into the cell and ( ii ) a decrease in PK that may be due to a direct effect on the calcium-sensitive PK itself .
	manualset3
106305	11	401801	13	NULL	NULL	0	NULL	calcium-sensitive PK 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that tolbutamide has two opposing actions on islet beta-cell 86Rb efflux , and therefore PK : ( i ) a tendency to increase a calcium-sensitive PK by stimulating calcium entry into the cell and ( ii ) a decrease in PK that may be due to a direct effect on the calcium-sensitive PK itself .
	manualset3
106306	1	401802	13	NULL	NULL	0	NULL	radical surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that too much radical surgery is being performed in patients who can be recognized preoperatively as having obviously advanced disease .
	manualset3
106307	2	401802	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that too much radical surgery is being performed in patients who can be recognized preoperatively as having obviously advanced disease .
	manualset3
106308	3	401802	13	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that too much radical surgery is being performed in patients who can be recognized preoperatively as having obviously advanced disease .
	manualset3
106309	1	401803	13	NULL	NULL	0	NULL	conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that under some conditions filling the vagina with air ( tightly ) can cause fatal air embolisms .
	manualset3
106310	2	401803	13	NULL	NULL	0	NULL	vagina	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that under some conditions filling the vagina with air ( tightly ) can cause fatal air embolisms .
	manualset3
106311	3	401803	13	NULL	NULL	0	NULL	air 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that under some conditions filling the vagina with air ( tightly ) can cause fatal air embolisms .
	manualset3
106312	4	401803	13	NULL	NULL	0	NULL	fatal air embolisms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that under some conditions filling the vagina with air ( tightly ) can cause fatal air embolisms .
	manualset3
106313	1	401804	13	NULL	NULL	0	NULL	implants	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It is conducted by placing implants at M2 and M2 areas of adult monkey .
	manualset3
106314	2	401804	13	NULL	NULL	NULL	NULL	M2 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is conducted by placing implants at M2 and M2 areas of adult monkey .
	manualset3
106315	3	401804	13	NULL	NULL	0	NULL	M2 areas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is conducted by placing implants at M2 and M2 areas of adult monkey .
	manualset3
106316	4	401804	13	NULL	NULL	0	NULL	 adult monkey	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It is conducted by placing implants at M2 and M2 areas of adult monkey .
	manualset3
106317	1	401805	13	NULL	NULL	0	NULL	60 specimens	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	60 specimens were taken for diagnostic sampling , 46 were taken during endoscopic laser resection , and 19 for overtly benign pathology .
	manualset3
106318	2	401805	13	NULL	NULL	0	NULL	diagnostic sampling 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	60 specimens were taken for diagnostic sampling , 46 were taken during endoscopic laser resection , and 19 for overtly benign pathology .
	manualset3
106319	3	401805	13	NULL	NULL	0	NULL	46	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	60 specimens were taken for diagnostic sampling , 46 were taken during endoscopic laser resection , and 19 for overtly benign pathology .
	manualset3
106320	4	401805	13	NULL	NULL	0	NULL	endoscopic laser resection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	60 specimens were taken for diagnostic sampling , 46 were taken during endoscopic laser resection , and 19 for overtly benign pathology .
	manualset3
106321	5	401805	13	NULL	NULL	0	NULL	19	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	60 specimens were taken for diagnostic sampling , 46 were taken during endoscopic laser resection , and 19 for overtly benign pathology .
	manualset3
106322	6	401805	13	NULL	NULL	0	NULL	benign pathology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	60 specimens were taken for diagnostic sampling , 46 were taken during endoscopic laser resection , and 19 for overtly benign pathology .
	manualset3
106323	1	401806	13	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is critical that the diagnosis is considered and confirmed promptly due to rapid deterioration and a potentially fatal outcome in the absence of aggressive treatment .
	manualset3
106324	2	401806	13	NULL	NULL	0	NULL	rapid deterioration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is critical that the diagnosis is considered and confirmed promptly due to rapid deterioration and a potentially fatal outcome in the absence of aggressive treatment .
	manualset3
106325	3	401806	13	NULL	NULL	0	NULL	fatal outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is critical that the diagnosis is considered and confirmed promptly due to rapid deterioration and a potentially fatal outcome in the absence of aggressive treatment .
	manualset3
106326	4	401806	13	NULL	NULL	0	NULL	 absence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is critical that the diagnosis is considered and confirmed promptly due to rapid deterioration and a potentially fatal outcome in the absence of aggressive treatment .
	manualset3
106327	5	401806	13	NULL	NULL	0	NULL	aggressive treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is critical that the diagnosis is considered and confirmed promptly due to rapid deterioration and a potentially fatal outcome in the absence of aggressive treatment .
	manualset3
106328	1	401807	13	NULL	NULL	0	NULL	burn institution	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It is crucial for every burn institution to determine the specific pattern of burn wound microbial colonization , the time-related changes in the dominant flora , and the antimicrobial sensitivity profiles .
	manualset3
106329	2	401807	13	NULL	NULL	0	NULL	specific pattern	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is crucial for every burn institution to determine the specific pattern of burn wound microbial colonization , the time-related changes in the dominant flora , and the antimicrobial sensitivity profiles .
	manualset3
106330	3	401807	13	NULL	NULL	0	NULL	burn wound microbial colonization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is crucial for every burn institution to determine the specific pattern of burn wound microbial colonization , the time-related changes in the dominant flora , and the antimicrobial sensitivity profiles .
	manualset3
106331	4	401807	13	NULL	NULL	0	NULL	time-related changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is crucial for every burn institution to determine the specific pattern of burn wound microbial colonization , the time-related changes in the dominant flora , and the antimicrobial sensitivity profiles .
	manualset3
106332	5	401807	13	NULL	NULL	0	NULL	dominant flora	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It is crucial for every burn institution to determine the specific pattern of burn wound microbial colonization , the time-related changes in the dominant flora , and the antimicrobial sensitivity profiles .
	manualset3
106333	6	401807	13	NULL	NULL	0	NULL	antimicrobial sensitivity profiles	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is crucial for every burn institution to determine the specific pattern of burn wound microbial colonization , the time-related changes in the dominant flora , and the antimicrobial sensitivity profiles .
	manualset3
106334	1	401808	13	NULL	NULL	0	NULL	urban flux	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is demonstrated that this extremely large and urban flux of fine sediment is likely to have a major downstream impact on water quality in the River Aire .
	manualset3
106335	2	401808	13	NULL	NULL	0	NULL	sediment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is demonstrated that this extremely large and urban flux of fine sediment is likely to have a major downstream impact on water quality in the River Aire .
	manualset3
106336	3	401808	13	NULL	NULL	0	NULL	downstream impact 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is demonstrated that this extremely large and urban flux of fine sediment is likely to have a major downstream impact on water quality in the River Aire .
	manualset3
106337	4	401808	13	NULL	NULL	0	NULL	water quality	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is demonstrated that this extremely large and urban flux of fine sediment is likely to have a major downstream impact on water quality in the River Aire .
	manualset3
106338	5	401808	13	NULL	NULL	0	NULL	 River Aire 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	It is demonstrated that this extremely large and urban flux of fine sediment is likely to have a major downstream impact on water quality in the River Aire .
	manualset3
106339	1	401809	13	NULL	NULL	0	NULL	people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is emphasized that some people living at home with relatives also have chronic mental disabilities as have a high proportion of the destitute .
	manualset3
106340	2	401809	13	NULL	NULL	0	NULL	home	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It is emphasized that some people living at home with relatives also have chronic mental disabilities as have a high proportion of the destitute .
	manualset3
106341	3	401809	13	NULL	NULL	0	NULL	relatives	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is emphasized that some people living at home with relatives also have chronic mental disabilities as have a high proportion of the destitute .
	manualset3
106342	4	401809	13	NULL	NULL	0	NULL	chronic mental disabilities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is emphasized that some people living at home with relatives also have chronic mental disabilities as have a high proportion of the destitute .
	manualset3
106343	5	401809	13	NULL	NULL	0	NULL	 high proportion	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is emphasized that some people living at home with relatives also have chronic mental disabilities as have a high proportion of the destitute .
	manualset3
106344	1	401810	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	It is evident from the study that leisure intervention groups facilitate both leisure satisfaction and improved quality of life .
	manualset3
106345	2	401810	13	NULL	NULL	0	NULL	leisure intervention groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is evident from the study that leisure intervention groups facilitate both leisure satisfaction and improved quality of life .
	manualset3
106346	3	401810	13	NULL	NULL	0	NULL	leisure satisfaction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is evident from the study that leisure intervention groups facilitate both leisure satisfaction and improved quality of life .
	manualset3
106347	4	401810	13	NULL	NULL	0	NULL	quality of life 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is evident from the study that leisure intervention groups facilitate both leisure satisfaction and improved quality of life .
	manualset3
106348	1	401811	13	NULL	NULL	0	NULL	COUP-TFII	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is first confirmed that COUP-TFII is expressed in VEC but not in AEC in the adult .
	manualset3
106349	2	401811	13	NULL	NULL	0	NULL	VEC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It is first confirmed that COUP-TFII is expressed in VEC but not in AEC in the adult .
	manualset3
106350	3	401811	13	NULL	NULL	0	NULL	AEC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It is first confirmed that COUP-TFII is expressed in VEC but not in AEC in the adult .
	manualset3
106351	4	401811	13	NULL	NULL	NULL	NULL	adult 	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is first confirmed that COUP-TFII is expressed in VEC but not in AEC in the adult .
	manualset3
106352	1	401812	13	NULL	NULL	0	NULL	62	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	62 patients ( 64 hips , mean age 56 years , range : 32-75 ) were randomized to porous Trilogy cups with ( 30 ) and without ( 34 ) cluster holes for additional screw fixation .
	manualset3
106353	2	401812	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	62 patients ( 64 hips , mean age 56 years , range : 32-75 ) were randomized to porous Trilogy cups with ( 30 ) and without ( 34 ) cluster holes for additional screw fixation .
	manualset3
106354	3	401812	13	NULL	NULL	0	NULL	64	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	62 patients ( 64 hips , mean age 56 years , range : 32-75 ) were randomized to porous Trilogy cups with ( 30 ) and without ( 34 ) cluster holes for additional screw fixation .
	manualset3
106355	4	401812	13	NULL	NULL	0	NULL	hips	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	62 patients ( 64 hips , mean age 56 years , range : 32-75 ) were randomized to porous Trilogy cups with ( 30 ) and without ( 34 ) cluster holes for additional screw fixation .
	manualset3
106356	5	401812	13	NULL	NULL	NULL	NULL	mean age 56 years	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	62 patients ( 64 hips , mean age 56 years , range : 32-75 ) were randomized to porous Trilogy cups with ( 30 ) and without ( 34 ) cluster holes for additional screw fixation .
	manualset3
106357	6	401812	13	NULL	NULL	0	NULL	range : 32-75	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	62 patients ( 64 hips , mean age 56 years , range : 32-75 ) were randomized to porous Trilogy cups with ( 30 ) and without ( 34 ) cluster holes for additional screw fixation .
	manualset3
106358	7	401812	13	NULL	NULL	0	NULL	porous Trilogy cups	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	62 patients ( 64 hips , mean age 56 years , range : 32-75 ) were randomized to porous Trilogy cups with ( 30 ) and without ( 34 ) cluster holes for additional screw fixation .
	manualset3
106360	9	401812	13	NULL	NULL	0	NULL	30 cluster holes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	62 patients ( 64 hips , mean age 56 years , range : 32-75 ) were randomized to porous Trilogy cups with ( 30 ) and without ( 34 ) cluster holes for additional screw fixation .
	manualset3
106361	10	401812	13	NULL	NULL	0	NULL	( 34 ) cluster holes 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	62 patients ( 64 hips , mean age 56 years , range : 32-75 ) were randomized to porous Trilogy cups with ( 30 ) and without ( 34 ) cluster holes for additional screw fixation .
	manualset3
106362	11	401812	13	NULL	NULL	0	NULL	screw fixation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	62 patients ( 64 hips , mean age 56 years , range : 32-75 ) were randomized to porous Trilogy cups with ( 30 ) and without ( 34 ) cluster holes for additional screw fixation .
	manualset3
106363	1	401813	13	NULL	NULL	0	NULL	acetonitrile	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is found that acetonitrile is mainly responsible for the good resolution of PEGylated proteins with the help of PEO coating in the semi-aqueous system .
	manualset3
106364	2	401813	13	NULL	NULL	0	NULL	resolution	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is found that acetonitrile is mainly responsible for the good resolution of PEGylated proteins with the help of PEO coating in the semi-aqueous system .
	manualset3
106365	3	401813	13	NULL	NULL	NULL	NULL	PEGylated proteins 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is found that acetonitrile is mainly responsible for the good resolution of PEGylated proteins with the help of PEO coating in the semi-aqueous system .
	manualset3
106366	4	401813	13	NULL	NULL	0	NULL	PEO coating	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	It is found that acetonitrile is mainly responsible for the good resolution of PEGylated proteins with the help of PEO coating in the semi-aqueous system .
	manualset3
106367	5	401813	13	NULL	NULL	0	NULL	semi-aqueous system 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	It is found that acetonitrile is mainly responsible for the good resolution of PEGylated proteins with the help of PEO coating in the semi-aqueous system .
	manualset3
106368	1	401814	13	NULL	NULL	0	NULL	conformational changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is found that the conformational changes are converted to changes in the electrostatic interaction between the protein and its ligands , which drives the ATP synthesis .
	manualset3
106369	2	401814	13	NULL	NULL	0	NULL	changes 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is found that the conformational changes are converted to changes in the electrostatic interaction between the protein and its ligands , which drives the ATP synthesis .
	manualset3
106370	3	401814	13	NULL	NULL	0	NULL	electrostatic interaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is found that the conformational changes are converted to changes in the electrostatic interaction between the protein and its ligands , which drives the ATP synthesis .
	manualset3
106371	4	401814	13	NULL	NULL	0	NULL	 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is found that the conformational changes are converted to changes in the electrostatic interaction between the protein and its ligands , which drives the ATP synthesis .
	manualset3
106372	5	401814	13	NULL	NULL	0	NULL	ligands	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is found that the conformational changes are converted to changes in the electrostatic interaction between the protein and its ligands , which drives the ATP synthesis .
	manualset3
106373	6	401814	13	NULL	NULL	0	NULL	ATP synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is found that the conformational changes are converted to changes in the electrostatic interaction between the protein and its ligands , which drives the ATP synthesis .
	manualset3
106374	1	401815	13	NULL	NULL	0	NULL	skier 's 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	It is found that the skier 's postures , wind speed , and direction play a significant role .
	manualset3
106375	2	401815	13	NULL	NULL	NULL	NULL	postures	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is found that the skier 's postures , wind speed , and direction play a significant role .
	manualset3
106376	3	401815	13	NULL	NULL	0	NULL	wind speed	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is found that the skier 's postures , wind speed , and direction play a significant role .
	manualset3
106377	4	401815	13	NULL	NULL	0	NULL	direction play	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is found that the skier 's postures , wind speed , and direction play a significant role .
	manualset3
106378	5	401815	13	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is found that the skier 's postures , wind speed , and direction play a significant role .
	manualset3
106379	1	401816	13	NULL	NULL	0	NULL	 addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is hoped that the addition of these groups will help to improve overall treatment outcome of the clients who are served by the agency .
	manualset3
106380	2	401816	13	NULL	NULL	0	NULL	groups 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is hoped that the addition of these groups will help to improve overall treatment outcome of the clients who are served by the agency .
	manualset3
106381	3	401816	13	NULL	NULL	0	NULL	treatment outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is hoped that the addition of these groups will help to improve overall treatment outcome of the clients who are served by the agency .
	manualset3
106382	4	401816	13	NULL	NULL	0	NULL	clients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is hoped that the addition of these groups will help to improve overall treatment outcome of the clients who are served by the agency .
	manualset3
106383	5	401816	13	NULL	NULL	0	NULL	agency	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is hoped that the addition of these groups will help to improve overall treatment outcome of the clients who are served by the agency .
	manualset3
106384	1	401817	13	NULL	NULL	0	NULL	sine-wave replicas	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	It is hypothesized that in sine-wave replicas of natural speech , lexical tone recognition would be severely impaired due to the loss of F0 information , but the linguistic information at the sentence level could be retrieved even with limited tone information .
	manualset3
106385	2	401817	13	NULL	NULL	0	NULL	natural speech	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is hypothesized that in sine-wave replicas of natural speech , lexical tone recognition would be severely impaired due to the loss of F0 information , but the linguistic information at the sentence level could be retrieved even with limited tone information .
	manualset3
106386	3	401817	13	NULL	NULL	0	NULL	lexical tone recognition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is hypothesized that in sine-wave replicas of natural speech , lexical tone recognition would be severely impaired due to the loss of F0 information , but the linguistic information at the sentence level could be retrieved even with limited tone information .
	manualset3
106387	4	401817	13	NULL	NULL	0	NULL	loss	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is hypothesized that in sine-wave replicas of natural speech , lexical tone recognition would be severely impaired due to the loss of F0 information , but the linguistic information at the sentence level could be retrieved even with limited tone information .
	manualset3
106388	5	401817	13	NULL	NULL	0	NULL	F0 information 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is hypothesized that in sine-wave replicas of natural speech , lexical tone recognition would be severely impaired due to the loss of F0 information , but the linguistic information at the sentence level could be retrieved even with limited tone information .
	manualset3
106389	6	401817	13	NULL	NULL	0	NULL	linguistic information	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is hypothesized that in sine-wave replicas of natural speech , lexical tone recognition would be severely impaired due to the loss of F0 information , but the linguistic information at the sentence level could be retrieved even with limited tone information .
	manualset3
106390	7	401817	13	NULL	NULL	0	NULL	sentence level	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is hypothesized that in sine-wave replicas of natural speech , lexical tone recognition would be severely impaired due to the loss of F0 information , but the linguistic information at the sentence level could be retrieved even with limited tone information .
	manualset3
106391	8	401817	13	NULL	NULL	0	NULL	 tone information	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is hypothesized that in sine-wave replicas of natural speech , lexical tone recognition would be severely impaired due to the loss of F0 information , but the linguistic information at the sentence level could be retrieved even with limited tone information .
	manualset3
106392	1	401818	13	NULL	NULL	0	NULL	nursing practice 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is important to evaluate nursing practice within the specific cultural context before applying terminology and meaning of concepts used .
	manualset3
106393	2	401818	13	NULL	NULL	0	NULL	cultural context	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is important to evaluate nursing practice within the specific cultural context before applying terminology and meaning of concepts used .
	manualset3
106394	3	401818	13	NULL	NULL	0	NULL	terminology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	It is important to evaluate nursing practice within the specific cultural context before applying terminology and meaning of concepts used .
	manualset3
106395	4	401818	13	NULL	NULL	0	NULL	meaning of concepts	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	It is important to evaluate nursing practice within the specific cultural context before applying terminology and meaning of concepts used .
	manualset3
106396	1	401819	13	NULL	NULL	0	NULL	 family	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is important to reassure the family that the lesions will disappear with time .
	manualset3
106397	2	401819	13	NULL	NULL	0	NULL	lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is important to reassure the family that the lesions will disappear with time .
	manualset3
106398	3	401819	13	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	It is important to reassure the family that the lesions will disappear with time .
	manualset3
106399	1	401820	13	NULL	NULL	0	NULL	store	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is important to set great store by the physical examination ( which is often performed cursorily before the patients are referred to curative inpatients treatment ) , including a neurological examination and in some cases also EMG , special radiographs , myelography , CT , magnetic resonance imaging and the like to gather more information on the real cause of the low back pain .
	manualset3
106400	2	401820	13	NULL	NULL	0	NULL	physical examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is important to set great store by the physical examination ( which is often performed cursorily before the patients are referred to curative inpatients treatment ) , including a neurological examination and in some cases also EMG , special radiographs , myelography , CT , magnetic resonance imaging and the like to gather more information on the real cause of the low back pain .
	manualset3
106401	3	401820	13	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is important to set great store by the physical examination ( which is often performed cursorily before the patients are referred to curative inpatients treatment ) , including a neurological examination and in some cases also EMG , special radiographs , myelography , CT , magnetic resonance imaging and the like to gather more information on the real cause of the low back pain .
	manualset3
106402	4	401820	13	NULL	NULL	0	NULL	curative inpatients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is important to set great store by the physical examination ( which is often performed cursorily before the patients are referred to curative inpatients treatment ) , including a neurological examination and in some cases also EMG , special radiographs , myelography , CT , magnetic resonance imaging and the like to gather more information on the real cause of the low back pain .
	manualset3
106403	5	401820	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is important to set great store by the physical examination ( which is often performed cursorily before the patients are referred to curative inpatients treatment ) , including a neurological examination and in some cases also EMG , special radiographs , myelography , CT , magnetic resonance imaging and the like to gather more information on the real cause of the low back pain .
	manualset3
106404	6	401820	13	NULL	NULL	0	NULL	neurological examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is important to set great store by the physical examination ( which is often performed cursorily before the patients are referred to curative inpatients treatment ) , including a neurological examination and in some cases also EMG , special radiographs , myelography , CT , magnetic resonance imaging and the like to gather more information on the real cause of the low back pain .
	manualset3
106405	7	401820	13	NULL	NULL	0	NULL	 cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is important to set great store by the physical examination ( which is often performed cursorily before the patients are referred to curative inpatients treatment ) , including a neurological examination and in some cases also EMG , special radiographs , myelography , CT , magnetic resonance imaging and the like to gather more information on the real cause of the low back pain .
	manualset3
106406	8	401820	13	NULL	NULL	0	NULL	EMG	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is important to set great store by the physical examination ( which is often performed cursorily before the patients are referred to curative inpatients treatment ) , including a neurological examination and in some cases also EMG , special radiographs , myelography , CT , magnetic resonance imaging and the like to gather more information on the real cause of the low back pain .
	manualset3
106407	9	401820	13	NULL	NULL	0	NULL	special radiographs 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is important to set great store by the physical examination ( which is often performed cursorily before the patients are referred to curative inpatients treatment ) , including a neurological examination and in some cases also EMG , special radiographs , myelography , CT , magnetic resonance imaging and the like to gather more information on the real cause of the low back pain .
	manualset3
106408	10	401820	13	NULL	NULL	0	NULL	myelography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is important to set great store by the physical examination ( which is often performed cursorily before the patients are referred to curative inpatients treatment ) , including a neurological examination and in some cases also EMG , special radiographs , myelography , CT , magnetic resonance imaging and the like to gather more information on the real cause of the low back pain .
	manualset3
106409	11	401820	13	NULL	NULL	0	NULL	CT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is important to set great store by the physical examination ( which is often performed cursorily before the patients are referred to curative inpatients treatment ) , including a neurological examination and in some cases also EMG , special radiographs , myelography , CT , magnetic resonance imaging and the like to gather more information on the real cause of the low back pain .
	manualset3
106410	12	401820	13	NULL	NULL	0	NULL	magnetic resonance imaging 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is important to set great store by the physical examination ( which is often performed cursorily before the patients are referred to curative inpatients treatment ) , including a neurological examination and in some cases also EMG , special radiographs , myelography , CT , magnetic resonance imaging and the like to gather more information on the real cause of the low back pain .
	manualset3
106411	13	401820	13	NULL	NULL	0	NULL	 information	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is important to set great store by the physical examination ( which is often performed cursorily before the patients are referred to curative inpatients treatment ) , including a neurological examination and in some cases also EMG , special radiographs , myelography , CT , magnetic resonance imaging and the like to gather more information on the real cause of the low back pain .
	manualset3
106412	14	401820	13	NULL	NULL	0	NULL	real cause 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is important to set great store by the physical examination ( which is often performed cursorily before the patients are referred to curative inpatients treatment ) , including a neurological examination and in some cases also EMG , special radiographs , myelography , CT , magnetic resonance imaging and the like to gather more information on the real cause of the low back pain .
	manualset3
106413	15	401820	13	NULL	NULL	0	NULL	low back pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is important to set great store by the physical examination ( which is often performed cursorily before the patients are referred to curative inpatients treatment ) , including a neurological examination and in some cases also EMG , special radiographs , myelography , CT , magnetic resonance imaging and the like to gather more information on the real cause of the low back pain .
	manualset3
106414	1	401821	13	NULL	NULL	0	NULL	63-70	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	63-70 , 1989 ) recently used an equation to calculate TP based on the consideration that it is about 95 % of the maximal SAP .
	manualset3
106415	2	401821	13	NULL	NULL	0	NULL	1989	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	63-70 , 1989 ) recently used an equation to calculate TP based on the consideration that it is about 95 % of the maximal SAP .
	manualset3
106416	3	401821	13	NULL	NULL	0	NULL	equation	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	63-70 , 1989 ) recently used an equation to calculate TP based on the consideration that it is about 95 % of the maximal SAP .
	manualset3
106417	4	401821	13	NULL	NULL	0	NULL	TP	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	63-70 , 1989 ) recently used an equation to calculate TP based on the consideration that it is about 95 % of the maximal SAP .
	manualset3
106418	5	401821	13	NULL	NULL	0	NULL	consideration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	63-70 , 1989 ) recently used an equation to calculate TP based on the consideration that it is about 95 % of the maximal SAP .
	manualset3
106419	6	401821	13	NULL	NULL	0	NULL	95 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	63-70 , 1989 ) recently used an equation to calculate TP based on the consideration that it is about 95 % of the maximal SAP .
	manualset3
106420	7	401821	13	NULL	NULL	0	NULL	maximal SAP	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	63-70 , 1989 ) recently used an equation to calculate TP based on the consideration that it is about 95 % of the maximal SAP .
	manualset3
106421	1	401822	13	NULL	NULL	0	NULL	thermolabile protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is induced by a thermolabile protein produced during the antiallograft immune response with a molecular weight of about 150 , 000 .
	manualset3
106422	2	401822	13	NULL	NULL	0	NULL	antiallograft immune response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is induced by a thermolabile protein produced during the antiallograft immune response with a molecular weight of about 150 , 000 .
	manualset3
106423	3	401822	13	NULL	NULL	0	NULL	molecular weight of about 150 , 000	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is induced by a thermolabile protein produced during the antiallograft immune response with a molecular weight of about 150 , 000 .
	manualset3
106424	1	401823	13	NULL	NULL	0	NULL	pectic catabolic products 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is induced by pectic catabolic products and affected by growth phase , temperature , iron starvation , osmolarity , anaerobiosis , nitrogen starvation and catabolite repression .
	manualset3
106425	2	401823	13	NULL	NULL	0	NULL	growth phase	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	It is induced by pectic catabolic products and affected by growth phase , temperature , iron starvation , osmolarity , anaerobiosis , nitrogen starvation and catabolite repression .
	manualset3
106426	3	401823	13	NULL	NULL	0	NULL	temperature	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	It is induced by pectic catabolic products and affected by growth phase , temperature , iron starvation , osmolarity , anaerobiosis , nitrogen starvation and catabolite repression .
	manualset3
106427	4	401823	13	NULL	NULL	0	NULL	 iron starvation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is induced by pectic catabolic products and affected by growth phase , temperature , iron starvation , osmolarity , anaerobiosis , nitrogen starvation and catabolite repression .
	manualset3
106428	5	401823	13	NULL	NULL	0	NULL	osmolarity 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is induced by pectic catabolic products and affected by growth phase , temperature , iron starvation , osmolarity , anaerobiosis , nitrogen starvation and catabolite repression .
	manualset3
106429	6	401823	13	NULL	NULL	0	NULL	anaerobiosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is induced by pectic catabolic products and affected by growth phase , temperature , iron starvation , osmolarity , anaerobiosis , nitrogen starvation and catabolite repression .
	manualset3
106430	7	401823	13	NULL	NULL	0	NULL	nitrogen starvation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is induced by pectic catabolic products and affected by growth phase , temperature , iron starvation , osmolarity , anaerobiosis , nitrogen starvation and catabolite repression .
	manualset3
106431	8	401823	13	NULL	NULL	0	NULL	catabolite repression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is induced by pectic catabolic products and affected by growth phase , temperature , iron starvation , osmolarity , anaerobiosis , nitrogen starvation and catabolite repression .
	manualset3
106432	1	401824	13	NULL	NULL	0	NULL	awareness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is intended to raise awareness and encourage implementation of preventive strategies in hepatology .
	manualset3
106433	2	401824	13	NULL	NULL	0	NULL	 implementation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is intended to raise awareness and encourage implementation of preventive strategies in hepatology .
	manualset3
106434	3	401824	13	NULL	NULL	0	NULL	preventive strategies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is intended to raise awareness and encourage implementation of preventive strategies in hepatology .
	manualset3
106435	4	401824	13	NULL	NULL	NULL	NULL	hepatology 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is intended to raise awareness and encourage implementation of preventive strategies in hepatology .
	manualset3
106436	1	401825	13	NULL	NULL	0	NULL	DNA damage 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is known that DNA damage causes the supernumerary centrosomes by a mechanism in which centrosomes continue to duplicate during cell cycle arrest at checkpoints .
	manualset3
106437	2	401825	13	NULL	NULL	0	NULL	 supernumerary centrosomes 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	It is known that DNA damage causes the supernumerary centrosomes by a mechanism in which centrosomes continue to duplicate during cell cycle arrest at checkpoints .
	manualset3
106438	3	401825	13	NULL	NULL	0	NULL	mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is known that DNA damage causes the supernumerary centrosomes by a mechanism in which centrosomes continue to duplicate during cell cycle arrest at checkpoints .
	manualset3
106439	4	401825	13	NULL	NULL	0	NULL	centrosomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	It is known that DNA damage causes the supernumerary centrosomes by a mechanism in which centrosomes continue to duplicate during cell cycle arrest at checkpoints .
	manualset3
106440	5	401825	13	NULL	NULL	0	NULL	cell cycle arrest	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is known that DNA damage causes the supernumerary centrosomes by a mechanism in which centrosomes continue to duplicate during cell cycle arrest at checkpoints .
	manualset3
106441	6	401825	13	NULL	NULL	0	NULL	checkpoints 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is known that DNA damage causes the supernumerary centrosomes by a mechanism in which centrosomes continue to duplicate during cell cycle arrest at checkpoints .
	manualset3
106442	1	401826	13	NULL	NULL	0	NULL	complexes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is known that complexes of DNA with histones and other proteins of apoptotic cells are the primary immunogens in systemic lupus erythematosus ( SLE ) .
	manualset3
106443	2	401826	13	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It is known that complexes of DNA with histones and other proteins of apoptotic cells are the primary immunogens in systemic lupus erythematosus ( SLE ) .
	manualset3
106444	3	401826	13	NULL	NULL	0	NULL	 histones	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is known that complexes of DNA with histones and other proteins of apoptotic cells are the primary immunogens in systemic lupus erythematosus ( SLE ) .
	manualset3
106445	4	401826	13	NULL	NULL	0	NULL	proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is known that complexes of DNA with histones and other proteins of apoptotic cells are the primary immunogens in systemic lupus erythematosus ( SLE ) .
	manualset3
106446	5	401826	13	NULL	NULL	0	NULL	apoptotic cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It is known that complexes of DNA with histones and other proteins of apoptotic cells are the primary immunogens in systemic lupus erythematosus ( SLE ) .
	manualset3
106447	6	401826	13	NULL	NULL	0	NULL	primary immunogens	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is known that complexes of DNA with histones and other proteins of apoptotic cells are the primary immunogens in systemic lupus erythematosus ( SLE ) .
	manualset3
106448	7	401826	13	NULL	NULL	0	NULL	systemic lupus erythematosus ( SLE ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It is known that complexes of DNA with histones and other proteins of apoptotic cells are the primary immunogens in systemic lupus erythematosus ( SLE ) .
	manualset3
106449	1	401827	13	NULL	NULL	0	NULL	arc welding pool	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	It is known that the arc welding pool temperature is related to the weld penetration depth ; therefore , by monitoring the temperature , the arc pool temperature and penetration depth are also monitored .
	manualset3
106450	2	401827	13	NULL	NULL	0	NULL	temperature 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	It is known that the arc welding pool temperature is related to the weld penetration depth ; therefore , by monitoring the temperature , the arc pool temperature and penetration depth are also monitored .
	manualset3
106451	3	401827	13	NULL	NULL	NULL	NULL	penetration depth	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is known that the arc welding pool temperature is related to the weld penetration depth ; therefore , by monitoring the temperature , the arc pool temperature and penetration depth are also monitored .
	manualset3
106452	4	401827	13	NULL	NULL	0	NULL	temperature	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	It is known that the arc welding pool temperature is related to the weld penetration depth ; therefore , by monitoring the temperature , the arc pool temperature and penetration depth are also monitored .
	manualset3
106453	5	401827	13	NULL	NULL	0	NULL	arc pool temperature	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	It is known that the arc welding pool temperature is related to the weld penetration depth ; therefore , by monitoring the temperature , the arc pool temperature and penetration depth are also monitored .
	manualset3
106454	6	401827	13	NULL	NULL	0	NULL	penetration depth	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is known that the arc welding pool temperature is related to the weld penetration depth ; therefore , by monitoring the temperature , the arc pool temperature and penetration depth are also monitored .
	manualset3
106455	1	401828	13	NULL	NULL	0	NULL	hair cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It is known that the outer hair cells are selectively protected by sound-conditioning .
	manualset3
106456	2	401828	13	NULL	NULL	0	NULL	sound-conditioning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is known that the outer hair cells are selectively protected by sound-conditioning .
	manualset3
106457	1	401829	13	NULL	NULL	0	NULL	azelastine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	It is likely that azelastine is able to inhibit bronchial hyperresponsiveness to chemical mediators of bronchial asthma .
	manualset3
106458	2	401829	13	NULL	NULL	0	NULL	bronchial hyperresponsiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is likely that azelastine is able to inhibit bronchial hyperresponsiveness to chemical mediators of bronchial asthma .
	manualset3
106459	3	401829	13	NULL	NULL	0	NULL	chemical mediators	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is likely that azelastine is able to inhibit bronchial hyperresponsiveness to chemical mediators of bronchial asthma .
	manualset3
106460	4	401829	13	NULL	NULL	0	NULL	bronchial asthma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It is likely that azelastine is able to inhibit bronchial hyperresponsiveness to chemical mediators of bronchial asthma .
	manualset3
106461	1	401830	13	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It is likely that the increasing number of seropositive women will be reflected in an increase in the number of reports of perinatal HIV infection and AIDS .
	manualset3
106462	2	401830	13	NULL	NULL	0	NULL	seropositive women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is likely that the increasing number of seropositive women will be reflected in an increase in the number of reports of perinatal HIV infection and AIDS .
	manualset3
106463	3	401830	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is likely that the increasing number of seropositive women will be reflected in an increase in the number of reports of perinatal HIV infection and AIDS .
	manualset3
106464	4	401830	13	NULL	NULL	0	NULL	number of reports	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It is likely that the increasing number of seropositive women will be reflected in an increase in the number of reports of perinatal HIV infection and AIDS .
	manualset3
106465	5	401830	13	NULL	NULL	0	NULL	perinatal HIV infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is likely that the increasing number of seropositive women will be reflected in an increase in the number of reports of perinatal HIV infection and AIDS .
	manualset3
106466	6	401830	13	NULL	NULL	0	NULL	AIDS 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is likely that the increasing number of seropositive women will be reflected in an increase in the number of reports of perinatal HIV infection and AIDS .
	manualset3
106689	1	401831	13	NULL	NULL	0	NULL	65	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	65 patients belonging to known acquired-immune-deficiency-syndrome ( AIDS ) risk groups were tested for mitogen responsiveness to pokeweed mitogen , concanavalin A and phytohemagglutinin , percentages of peripheral blood CD4 , CD8 and Leu7 lymphocyte subsets , serum neopterin levels , and gamma-interferon ( gamma-IFN ) concentrations in cell culture supernatants .
	manualset3
106690	2	401831	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	65 patients belonging to known acquired-immune-deficiency-syndrome ( AIDS ) risk groups were tested for mitogen responsiveness to pokeweed mitogen , concanavalin A and phytohemagglutinin , percentages of peripheral blood CD4 , CD8 and Leu7 lymphocyte subsets , serum neopterin levels , and gamma-interferon ( gamma-IFN ) concentrations in cell culture supernatants .
	manualset3
106692	3	401831	13	NULL	NULL	NULL	NULL	acquired-immune-deficiency-syndrome ( AIDS )	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	65 patients belonging to known acquired-immune-deficiency-syndrome ( AIDS ) risk groups were tested for mitogen responsiveness to pokeweed mitogen , concanavalin A and phytohemagglutinin , percentages of peripheral blood CD4 , CD8 and Leu7 lymphocyte subsets , serum neopterin levels , and gamma-interferon ( gamma-IFN ) concentrations in cell culture supernatants .
	manualset3
106693	4	401831	13	NULL	NULL	0	NULL	risk groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	65 patients belonging to known acquired-immune-deficiency-syndrome ( AIDS ) risk groups were tested for mitogen responsiveness to pokeweed mitogen , concanavalin A and phytohemagglutinin , percentages of peripheral blood CD4 , CD8 and Leu7 lymphocyte subsets , serum neopterin levels , and gamma-interferon ( gamma-IFN ) concentrations in cell culture supernatants .
	manualset3
106697	5	401831	13	NULL	NULL	0	NULL	mitogen responsiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	65 patients belonging to known acquired-immune-deficiency-syndrome ( AIDS ) risk groups were tested for mitogen responsiveness to pokeweed mitogen , concanavalin A and phytohemagglutinin , percentages of peripheral blood CD4 , CD8 and Leu7 lymphocyte subsets , serum neopterin levels , and gamma-interferon ( gamma-IFN ) concentrations in cell culture supernatants .
	manualset3
106699	6	401831	13	NULL	NULL	0	NULL	pokeweed mitogen	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	65 patients belonging to known acquired-immune-deficiency-syndrome ( AIDS ) risk groups were tested for mitogen responsiveness to pokeweed mitogen , concanavalin A and phytohemagglutinin , percentages of peripheral blood CD4 , CD8 and Leu7 lymphocyte subsets , serum neopterin levels , and gamma-interferon ( gamma-IFN ) concentrations in cell culture supernatants .
	manualset3
106701	7	401831	13	NULL	NULL	0	NULL	concanavalin A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	65 patients belonging to known acquired-immune-deficiency-syndrome ( AIDS ) risk groups were tested for mitogen responsiveness to pokeweed mitogen , concanavalin A and phytohemagglutinin , percentages of peripheral blood CD4 , CD8 and Leu7 lymphocyte subsets , serum neopterin levels , and gamma-interferon ( gamma-IFN ) concentrations in cell culture supernatants .
	manualset3
106703	8	401831	13	NULL	NULL	0	NULL	phytohemagglutinin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	65 patients belonging to known acquired-immune-deficiency-syndrome ( AIDS ) risk groups were tested for mitogen responsiveness to pokeweed mitogen , concanavalin A and phytohemagglutinin , percentages of peripheral blood CD4 , CD8 and Leu7 lymphocyte subsets , serum neopterin levels , and gamma-interferon ( gamma-IFN ) concentrations in cell culture supernatants .
	manualset3
106706	9	401831	13	NULL	NULL	0	NULL	percentages	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	65 patients belonging to known acquired-immune-deficiency-syndrome ( AIDS ) risk groups were tested for mitogen responsiveness to pokeweed mitogen , concanavalin A and phytohemagglutinin , percentages of peripheral blood CD4 , CD8 and Leu7 lymphocyte subsets , serum neopterin levels , and gamma-interferon ( gamma-IFN ) concentrations in cell culture supernatants .
	manualset3
106708	10	401831	13	NULL	NULL	0	NULL	 peripheral blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	65 patients belonging to known acquired-immune-deficiency-syndrome ( AIDS ) risk groups were tested for mitogen responsiveness to pokeweed mitogen , concanavalin A and phytohemagglutinin , percentages of peripheral blood CD4 , CD8 and Leu7 lymphocyte subsets , serum neopterin levels , and gamma-interferon ( gamma-IFN ) concentrations in cell culture supernatants .
	manualset3
106709	11	401831	13	NULL	NULL	0	NULL	CD4 lymphocyte subset	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	65 patients belonging to known acquired-immune-deficiency-syndrome ( AIDS ) risk groups were tested for mitogen responsiveness to pokeweed mitogen , concanavalin A and phytohemagglutinin , percentages of peripheral blood CD4 , CD8 and Leu7 lymphocyte subsets , serum neopterin levels , and gamma-interferon ( gamma-IFN ) concentrations in cell culture supernatants .
	manualset3
106710	12	401831	13	NULL	NULL	0	NULL	CD8 lymphocyte subset	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	65 patients belonging to known acquired-immune-deficiency-syndrome ( AIDS ) risk groups were tested for mitogen responsiveness to pokeweed mitogen , concanavalin A and phytohemagglutinin , percentages of peripheral blood CD4 , CD8 and Leu7 lymphocyte subsets , serum neopterin levels , and gamma-interferon ( gamma-IFN ) concentrations in cell culture supernatants .
	manualset3
106711	13	401831	13	NULL	NULL	0	NULL	Leu7 lymphocyte subset	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	65 patients belonging to known acquired-immune-deficiency-syndrome ( AIDS ) risk groups were tested for mitogen responsiveness to pokeweed mitogen , concanavalin A and phytohemagglutinin , percentages of peripheral blood CD4 , CD8 and Leu7 lymphocyte subsets , serum neopterin levels , and gamma-interferon ( gamma-IFN ) concentrations in cell culture supernatants .
	manualset3
106712	14	401831	13	NULL	NULL	0	NULL	serum neopterin levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	65 patients belonging to known acquired-immune-deficiency-syndrome ( AIDS ) risk groups were tested for mitogen responsiveness to pokeweed mitogen , concanavalin A and phytohemagglutinin , percentages of peripheral blood CD4 , CD8 and Leu7 lymphocyte subsets , serum neopterin levels , and gamma-interferon ( gamma-IFN ) concentrations in cell culture supernatants .
	manualset3
106713	15	401831	13	NULL	NULL	0	NULL	 gamma-interferon ( gamma-IFN )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	65 patients belonging to known acquired-immune-deficiency-syndrome ( AIDS ) risk groups were tested for mitogen responsiveness to pokeweed mitogen , concanavalin A and phytohemagglutinin , percentages of peripheral blood CD4 , CD8 and Leu7 lymphocyte subsets , serum neopterin levels , and gamma-interferon ( gamma-IFN ) concentrations in cell culture supernatants .
	manualset3
106714	16	401831	13	NULL	NULL	0	NULL	concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	65 patients belonging to known acquired-immune-deficiency-syndrome ( AIDS ) risk groups were tested for mitogen responsiveness to pokeweed mitogen , concanavalin A and phytohemagglutinin , percentages of peripheral blood CD4 , CD8 and Leu7 lymphocyte subsets , serum neopterin levels , and gamma-interferon ( gamma-IFN ) concentrations in cell culture supernatants .
	manualset3
106715	17	401831	13	NULL	NULL	0	NULL	cell culture supernatants	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	65 patients belonging to known acquired-immune-deficiency-syndrome ( AIDS ) risk groups were tested for mitogen responsiveness to pokeweed mitogen , concanavalin A and phytohemagglutinin , percentages of peripheral blood CD4 , CD8 and Leu7 lymphocyte subsets , serum neopterin levels , and gamma-interferon ( gamma-IFN ) concentrations in cell culture supernatants .
	manualset3
106716	1	401832	13	NULL	NULL	0	NULL	monitor	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is necessary to continuously monitor the molecular evolution and recombination events of EV71 .
	manualset3
106717	2	401832	13	NULL	NULL	0	NULL	molecular evolution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is necessary to continuously monitor the molecular evolution and recombination events of EV71 .
	manualset3
106718	3	401832	13	NULL	NULL	0	NULL	recombination events 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is necessary to continuously monitor the molecular evolution and recombination events of EV71 .
	manualset3
106720	4	401832	13	NULL	NULL	0	NULL	EV71 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It is necessary to continuously monitor the molecular evolution and recombination events of EV71 .
	manualset3
106723	1	401833	13	NULL	NULL	0	NULL	molecular drivers	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	It is necessary to identify the molecular drivers of these changes in bone turnover .
	manualset3
106724	2	401833	13	NULL	NULL	0	NULL	changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is necessary to identify the molecular drivers of these changes in bone turnover .
	manualset3
106725	3	401833	13	NULL	NULL	0	NULL	bone turnover 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is necessary to identify the molecular drivers of these changes in bone turnover .
	manualset3
106726	1	401834	13	NULL	NULL	0	NULL	secret	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is no secret that the accuracy of responses to items on the Outcome and Assessment Information Set ( OASIS ) varies greatly from clinician to clinician and item to item .
	manualset3
106727	2	401834	13	NULL	NULL	0	NULL	accuracy of responses 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is no secret that the accuracy of responses to items on the Outcome and Assessment Information Set ( OASIS ) varies greatly from clinician to clinician and item to item .
	manualset3
106728	3	401834	13	NULL	NULL	0	NULL	 items	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	It is no secret that the accuracy of responses to items on the Outcome and Assessment Information Set ( OASIS ) varies greatly from clinician to clinician and item to item .
	manualset3
106729	4	401834	13	NULL	NULL	0	NULL	Outcome and Assessment Information Set ( OASIS )	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is no secret that the accuracy of responses to items on the Outcome and Assessment Information Set ( OASIS ) varies greatly from clinician to clinician and item to item .
	manualset3
106730	5	401834	13	NULL	NULL	0	NULL	clinician	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	It is no secret that the accuracy of responses to items on the Outcome and Assessment Information Set ( OASIS ) varies greatly from clinician to clinician and item to item .
	manualset3
106731	6	401834	13	NULL	NULL	0	NULL	clinician	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	It is no secret that the accuracy of responses to items on the Outcome and Assessment Information Set ( OASIS ) varies greatly from clinician to clinician and item to item .
	manualset3
106732	7	401834	13	NULL	NULL	0	NULL	item	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	It is no secret that the accuracy of responses to items on the Outcome and Assessment Information Set ( OASIS ) varies greatly from clinician to clinician and item to item .
	manualset3
106733	8	401834	13	NULL	NULL	0	NULL	item	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	It is no secret that the accuracy of responses to items on the Outcome and Assessment Information Set ( OASIS ) varies greatly from clinician to clinician and item to item .
	manualset3
107008	1	401835	13	NULL	NULL	0	NULL	trivial question 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is not a trivial question whether the initial gain in efficiency will compensate for the lower information content in the plane integrals .
	manualset3
107009	2	401835	13	NULL	NULL	0	NULL	initial gain 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is not a trivial question whether the initial gain in efficiency will compensate for the lower information content in the plane integrals .
	manualset3
107010	3	401835	13	NULL	NULL	0	NULL	efficiency 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is not a trivial question whether the initial gain in efficiency will compensate for the lower information content in the plane integrals .
	manualset3
107011	4	401835	13	NULL	NULL	0	NULL	lower information content	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	It is not a trivial question whether the initial gain in efficiency will compensate for the lower information content in the plane integrals .
	manualset3
107012	5	401835	13	NULL	NULL	0	NULL	plane integrals 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is not a trivial question whether the initial gain in efficiency will compensate for the lower information content in the plane integrals .
	manualset3
107013	1	401836	13	NULL	NULL	0	NULL	CBF effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is not clear whether this CBF effect has a therapeutic role , but the impact of deep brain stimulation on cerebrovascular control warrants study from neuroscience , pathophysiological , and therapeutic perspectives .
	manualset3
107014	2	401836	13	NULL	NULL	0	NULL	therapeutic role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is not clear whether this CBF effect has a therapeutic role , but the impact of deep brain stimulation on cerebrovascular control warrants study from neuroscience , pathophysiological , and therapeutic perspectives .
	manualset3
107015	3	401836	13	NULL	NULL	0	NULL	 impact	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is not clear whether this CBF effect has a therapeutic role , but the impact of deep brain stimulation on cerebrovascular control warrants study from neuroscience , pathophysiological , and therapeutic perspectives .
	manualset3
107016	4	401836	13	NULL	NULL	NULL	NULL	deep brain stimulation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is not clear whether this CBF effect has a therapeutic role , but the impact of deep brain stimulation on cerebrovascular control warrants study from neuroscience , pathophysiological , and therapeutic perspectives .
	manualset3
107017	5	401836	13	NULL	NULL	NULL	NULL	cerebrovascular control	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is not clear whether this CBF effect has a therapeutic role , but the impact of deep brain stimulation on cerebrovascular control warrants study from neuroscience , pathophysiological , and therapeutic perspectives .
	manualset3
107018	6	401836	13	NULL	NULL	0	NULL	neuroscience perspective	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is not clear whether this CBF effect has a therapeutic role , but the impact of deep brain stimulation on cerebrovascular control warrants study from neuroscience , pathophysiological , and therapeutic perspectives .
	manualset3
107019	7	401836	13	NULL	NULL	0	NULL	pathophysiological perspective	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is not clear whether this CBF effect has a therapeutic role , but the impact of deep brain stimulation on cerebrovascular control warrants study from neuroscience , pathophysiological , and therapeutic perspectives .
	manualset3
107020	8	401836	13	NULL	NULL	0	NULL	therapeutic perspective	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is not clear whether this CBF effect has a therapeutic role , but the impact of deep brain stimulation on cerebrovascular control warrants study from neuroscience , pathophysiological , and therapeutic perspectives .
	manualset3
107021	1	401837	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is not known whether the increase in adiponectin during glitazone therapy is due to a suppression of ghrelin levels , a decrease of resistin concentrations or an amelioration of glucose control .
	manualset3
107022	2	401837	13	NULL	NULL	0	NULL	adiponectin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is not known whether the increase in adiponectin during glitazone therapy is due to a suppression of ghrelin levels , a decrease of resistin concentrations or an amelioration of glucose control .
	manualset3
107023	3	401837	13	NULL	NULL	0	NULL	glitazone therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is not known whether the increase in adiponectin during glitazone therapy is due to a suppression of ghrelin levels , a decrease of resistin concentrations or an amelioration of glucose control .
	manualset3
107024	4	401837	13	NULL	NULL	NULL	NULL	 suppression 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is not known whether the increase in adiponectin during glitazone therapy is due to a suppression of ghrelin levels , a decrease of resistin concentrations or an amelioration of glucose control .
	manualset3
107025	5	401837	13	NULL	NULL	0	NULL	ghrelin levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It is not known whether the increase in adiponectin during glitazone therapy is due to a suppression of ghrelin levels , a decrease of resistin concentrations or an amelioration of glucose control .
	manualset3
107026	6	401837	13	NULL	NULL	0	NULL	decrease	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is not known whether the increase in adiponectin during glitazone therapy is due to a suppression of ghrelin levels , a decrease of resistin concentrations or an amelioration of glucose control .
	manualset3
107027	7	401837	13	NULL	NULL	0	NULL	resistin concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It is not known whether the increase in adiponectin during glitazone therapy is due to a suppression of ghrelin levels , a decrease of resistin concentrations or an amelioration of glucose control .
	manualset3
107028	8	401837	13	NULL	NULL	0	NULL	glucose control	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is not known whether the increase in adiponectin during glitazone therapy is due to a suppression of ghrelin levels , a decrease of resistin concentrations or an amelioration of glucose control .
	manualset3
107029	1	401838	13	NULL	NULL	0	NULL	6th	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	6th diagnostic-therapeutic discourse of the ZFA in Freudenstadt 1975 ) .
	manualset3
107030	2	401838	13	NULL	NULL	0	NULL	diagnostic-therapeutic discourse	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	6th diagnostic-therapeutic discourse of the ZFA in Freudenstadt 1975 ) .
	manualset3
107031	3	401838	13	NULL	NULL	0	NULL	ZFA	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	6th diagnostic-therapeutic discourse of the ZFA in Freudenstadt 1975 ) .
	manualset3
107032	4	401838	13	NULL	NULL	0	NULL	 Freudenstadt 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	6th diagnostic-therapeutic discourse of the ZFA in Freudenstadt 1975 ) .
	manualset3
107033	5	401838	13	NULL	NULL	0	NULL	1975 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	6th diagnostic-therapeutic discourse of the ZFA in Freudenstadt 1975 ) .
	manualset3
107034	1	401839	13	NULL	NULL	0	NULL	lac promoter repression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is now appreciated that lac promoter repression involves cooperative binding of the bidentate lac repressor tetramer to pairs of lac operators via DNA looping .
	manualset3
107035	2	401839	13	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is now appreciated that lac promoter repression involves cooperative binding of the bidentate lac repressor tetramer to pairs of lac operators via DNA looping .
	manualset3
107036	3	401839	13	NULL	NULL	0	NULL	bidentate lac repressor tetramer 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It is now appreciated that lac promoter repression involves cooperative binding of the bidentate lac repressor tetramer to pairs of lac operators via DNA looping .
	manualset3
107037	4	401839	13	NULL	NULL	NULL	NULL	pairs of lac operators 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is now appreciated that lac promoter repression involves cooperative binding of the bidentate lac repressor tetramer to pairs of lac operators via DNA looping .
	manualset3
107038	5	401839	13	NULL	NULL	0	NULL	DNA looping	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is now appreciated that lac promoter repression involves cooperative binding of the bidentate lac repressor tetramer to pairs of lac operators via DNA looping .
	manualset3
107039	1	401840	13	NULL	NULL	0	NULL	IOP ( intraocular pression ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is now clear that IOP ( intraocular pression ) lowering treatment may significantly delay or prevent glaucoma development and progression .
	manualset3
107040	2	401840	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is now clear that IOP ( intraocular pression ) lowering treatment may significantly delay or prevent glaucoma development and progression .
	manualset3
107041	3	401840	13	NULL	NULL	0	NULL	glaucoma development	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is now clear that IOP ( intraocular pression ) lowering treatment may significantly delay or prevent glaucoma development and progression .
	manualset3
107042	4	401840	13	NULL	NULL	0	NULL	progression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is now clear that IOP ( intraocular pression ) lowering treatment may significantly delay or prevent glaucoma development and progression .
	manualset3
107043	1	401841	13	NULL	NULL	0	NULL	transformation-optical design	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	It is observed that a pure transformation-optical design can not result in a reflectionless beam expander/compressor .
	manualset3
107044	2	401841	13	NULL	NULL	0	NULL	beam expander/compressor	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It is observed that a pure transformation-optical design can not result in a reflectionless beam expander/compressor .
	manualset3
107045	1	401842	13	NULL	NULL	NULL	NULL	last 2 decades	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is only in the last 2 decades , however , that the powerful role exercise and physical activity play in treating and preventing type 2 diabetes has been fully appreciated .
	manualset3
107046	2	401842	13	NULL	NULL	NULL	NULL	powerful role exercise 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is only in the last 2 decades , however , that the powerful role exercise and physical activity play in treating and preventing type 2 diabetes has been fully appreciated .
	manualset3
107047	3	401842	13	NULL	NULL	0	NULL	physical activity play	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is only in the last 2 decades , however , that the powerful role exercise and physical activity play in treating and preventing type 2 diabetes has been fully appreciated .
	manualset3
107048	4	401842	13	NULL	NULL	0	NULL	type 2 diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It is only in the last 2 decades , however , that the powerful role exercise and physical activity play in treating and preventing type 2 diabetes has been fully appreciated .
	manualset3
107049	1	401843	13	NULL	NULL	0	NULL	teens	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is pointless to preach to teens about the evils of sex .
	manualset3
107050	2	401843	13	NULL	NULL	0	NULL	evils of sex 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is pointless to preach to teens about the evils of sex .
	manualset3
107051	1	401844	13	NULL	NULL	0	NULL	arterial dissecting aneurysms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is possible that some localized arterial dissecting aneurysms evolve to a localized aneurysmal sac , especially if they are located between Cl and the base of the skull .
	manualset3
107052	2	401844	13	NULL	NULL	0	NULL	aneurysmal sac 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is possible that some localized arterial dissecting aneurysms evolve to a localized aneurysmal sac , especially if they are located between Cl and the base of the skull .
	manualset3
107053	3	401844	13	NULL	NULL	0	NULL	Cl 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is possible that some localized arterial dissecting aneurysms evolve to a localized aneurysmal sac , especially if they are located between Cl and the base of the skull .
	manualset3
107054	4	401844	13	NULL	NULL	0	NULL	base of the skull 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is possible that some localized arterial dissecting aneurysms evolve to a localized aneurysmal sac , especially if they are located between Cl and the base of the skull .
	manualset3
107055	1	401845	13	NULL	NULL	0	NULL	phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is possible that the phosphorylation of c-ras p21 in CFC has a significant role in the growth factor-directed molecular cascade responsible for normal hemopoietic development .
	manualset3
107056	2	401845	13	NULL	NULL	0	NULL	c-ras p21 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is possible that the phosphorylation of c-ras p21 in CFC has a significant role in the growth factor-directed molecular cascade responsible for normal hemopoietic development .
	manualset3
107057	3	401845	13	NULL	NULL	0	NULL	CFC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It is possible that the phosphorylation of c-ras p21 in CFC has a significant role in the growth factor-directed molecular cascade responsible for normal hemopoietic development .
	manualset3
107058	4	401845	13	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is possible that the phosphorylation of c-ras p21 in CFC has a significant role in the growth factor-directed molecular cascade responsible for normal hemopoietic development .
	manualset3
107059	5	401845	13	NULL	NULL	0	NULL	growth factor-directed molecular cascade	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is possible that the phosphorylation of c-ras p21 in CFC has a significant role in the growth factor-directed molecular cascade responsible for normal hemopoietic development .
	manualset3
107060	6	401845	13	NULL	NULL	0	NULL	normal hemopoietic development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is possible that the phosphorylation of c-ras p21 in CFC has a significant role in the growth factor-directed molecular cascade responsible for normal hemopoietic development .
	manualset3
107061	1	401846	13	NULL	NULL	0	NULL	effective pore size distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is possible to determine an effective pore size distribution by fitting the capillary model to experimental breakthrough curves and pressure drop experiments .
	manualset3
107062	2	401846	13	NULL	NULL	0	NULL	capillary model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	It is possible to determine an effective pore size distribution by fitting the capillary model to experimental breakthrough curves and pressure drop experiments .
	manualset3
107063	3	401846	13	NULL	NULL	0	NULL	experimental breakthrough curves	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	It is possible to determine an effective pore size distribution by fitting the capillary model to experimental breakthrough curves and pressure drop experiments .
	manualset3
107064	4	401846	13	NULL	NULL	0	NULL	pressure drop experiments 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	It is possible to determine an effective pore size distribution by fitting the capillary model to experimental breakthrough curves and pressure drop experiments .
	manualset3
107065	1	401847	13	NULL	NULL	NULL	NULL	proteomic techniques 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is possible to use proteomic techniques to aid in detection , monitoring of treatment and progression , as well as gaining an increased understanding of cancer .
	manualset3
107066	2	401847	13	NULL	NULL	NULL	NULL	detection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is possible to use proteomic techniques to aid in detection , monitoring of treatment and progression , as well as gaining an increased understanding of cancer .
	manualset3
107067	3	401847	13	NULL	NULL	0	NULL	monitoring of treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is possible to use proteomic techniques to aid in detection , monitoring of treatment and progression , as well as gaining an increased understanding of cancer .
	manualset3
107068	4	401847	13	NULL	NULL	NULL	NULL	monitoring of progression	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is possible to use proteomic techniques to aid in detection , monitoring of treatment and progression , as well as gaining an increased understanding of cancer .
	manualset3
107069	5	401847	13	NULL	NULL	0	NULL	understanding of cancer	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is possible to use proteomic techniques to aid in detection , monitoring of treatment and progression , as well as gaining an increased understanding of cancer .
	manualset3
107070	1	401848	13	NULL	NULL	0	NULL	ability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that the ability to have survived the middle passage was positively correlated with greater responsiveness of the androgen receptor to its primary ligands dihydrotestosterone and testosterone , and that slaves possessing more responsive androgen receptors experienced a survival advantage engendered by the enhanced anabolic effects which accrued such as increased red cell mass and therefore greater oxygen carrying capacity and tissue oxygen delivery enabling these slaves to tolerate stifling conditions in the hull of the slave ship , increased lean muscle mass and therefore greater surface area to volume ratio resulting in easier ability to dissipate heat and remain cool , and increased skin thickness and sebum production resisting the macerating effect of lying in admixed bodily fluids below deck .
	manualset3
107071	2	401848	13	NULL	NULL	0	NULL	middle passage	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that the ability to have survived the middle passage was positively correlated with greater responsiveness of the androgen receptor to its primary ligands dihydrotestosterone and testosterone , and that slaves possessing more responsive androgen receptors experienced a survival advantage engendered by the enhanced anabolic effects which accrued such as increased red cell mass and therefore greater oxygen carrying capacity and tissue oxygen delivery enabling these slaves to tolerate stifling conditions in the hull of the slave ship , increased lean muscle mass and therefore greater surface area to volume ratio resulting in easier ability to dissipate heat and remain cool , and increased skin thickness and sebum production resisting the macerating effect of lying in admixed bodily fluids below deck .
	manualset3
107072	3	401848	13	NULL	NULL	0	NULL	greater responsiveness	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that the ability to have survived the middle passage was positively correlated with greater responsiveness of the androgen receptor to its primary ligands dihydrotestosterone and testosterone , and that slaves possessing more responsive androgen receptors experienced a survival advantage engendered by the enhanced anabolic effects which accrued such as increased red cell mass and therefore greater oxygen carrying capacity and tissue oxygen delivery enabling these slaves to tolerate stifling conditions in the hull of the slave ship , increased lean muscle mass and therefore greater surface area to volume ratio resulting in easier ability to dissipate heat and remain cool , and increased skin thickness and sebum production resisting the macerating effect of lying in admixed bodily fluids below deck .
	manualset3
107073	4	401848	13	NULL	NULL	0	NULL	androgen receptor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that the ability to have survived the middle passage was positively correlated with greater responsiveness of the androgen receptor to its primary ligands dihydrotestosterone and testosterone , and that slaves possessing more responsive androgen receptors experienced a survival advantage engendered by the enhanced anabolic effects which accrued such as increased red cell mass and therefore greater oxygen carrying capacity and tissue oxygen delivery enabling these slaves to tolerate stifling conditions in the hull of the slave ship , increased lean muscle mass and therefore greater surface area to volume ratio resulting in easier ability to dissipate heat and remain cool , and increased skin thickness and sebum production resisting the macerating effect of lying in admixed bodily fluids below deck .
	manualset3
107074	5	401848	13	NULL	NULL	0	NULL	primary ligands	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that the ability to have survived the middle passage was positively correlated with greater responsiveness of the androgen receptor to its primary ligands dihydrotestosterone and testosterone , and that slaves possessing more responsive androgen receptors experienced a survival advantage engendered by the enhanced anabolic effects which accrued such as increased red cell mass and therefore greater oxygen carrying capacity and tissue oxygen delivery enabling these slaves to tolerate stifling conditions in the hull of the slave ship , increased lean muscle mass and therefore greater surface area to volume ratio resulting in easier ability to dissipate heat and remain cool , and increased skin thickness and sebum production resisting the macerating effect of lying in admixed bodily fluids below deck .
	manualset3
107075	6	401848	13	NULL	NULL	0	NULL	dihydrotestosterone 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that the ability to have survived the middle passage was positively correlated with greater responsiveness of the androgen receptor to its primary ligands dihydrotestosterone and testosterone , and that slaves possessing more responsive androgen receptors experienced a survival advantage engendered by the enhanced anabolic effects which accrued such as increased red cell mass and therefore greater oxygen carrying capacity and tissue oxygen delivery enabling these slaves to tolerate stifling conditions in the hull of the slave ship , increased lean muscle mass and therefore greater surface area to volume ratio resulting in easier ability to dissipate heat and remain cool , and increased skin thickness and sebum production resisting the macerating effect of lying in admixed bodily fluids below deck .
	manualset3
107076	7	401848	13	NULL	NULL	0	NULL	testosterone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that the ability to have survived the middle passage was positively correlated with greater responsiveness of the androgen receptor to its primary ligands dihydrotestosterone and testosterone , and that slaves possessing more responsive androgen receptors experienced a survival advantage engendered by the enhanced anabolic effects which accrued such as increased red cell mass and therefore greater oxygen carrying capacity and tissue oxygen delivery enabling these slaves to tolerate stifling conditions in the hull of the slave ship , increased lean muscle mass and therefore greater surface area to volume ratio resulting in easier ability to dissipate heat and remain cool , and increased skin thickness and sebum production resisting the macerating effect of lying in admixed bodily fluids below deck .
	manualset3
107077	8	401848	13	NULL	NULL	0	NULL	slaves	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that the ability to have survived the middle passage was positively correlated with greater responsiveness of the androgen receptor to its primary ligands dihydrotestosterone and testosterone , and that slaves possessing more responsive androgen receptors experienced a survival advantage engendered by the enhanced anabolic effects which accrued such as increased red cell mass and therefore greater oxygen carrying capacity and tissue oxygen delivery enabling these slaves to tolerate stifling conditions in the hull of the slave ship , increased lean muscle mass and therefore greater surface area to volume ratio resulting in easier ability to dissipate heat and remain cool , and increased skin thickness and sebum production resisting the macerating effect of lying in admixed bodily fluids below deck .
	manualset3
107078	9	401848	13	NULL	NULL	0	NULL	androgen receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that the ability to have survived the middle passage was positively correlated with greater responsiveness of the androgen receptor to its primary ligands dihydrotestosterone and testosterone , and that slaves possessing more responsive androgen receptors experienced a survival advantage engendered by the enhanced anabolic effects which accrued such as increased red cell mass and therefore greater oxygen carrying capacity and tissue oxygen delivery enabling these slaves to tolerate stifling conditions in the hull of the slave ship , increased lean muscle mass and therefore greater surface area to volume ratio resulting in easier ability to dissipate heat and remain cool , and increased skin thickness and sebum production resisting the macerating effect of lying in admixed bodily fluids below deck .
	manualset3
107079	10	401848	13	NULL	NULL	0	NULL	survival advantage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that the ability to have survived the middle passage was positively correlated with greater responsiveness of the androgen receptor to its primary ligands dihydrotestosterone and testosterone , and that slaves possessing more responsive androgen receptors experienced a survival advantage engendered by the enhanced anabolic effects which accrued such as increased red cell mass and therefore greater oxygen carrying capacity and tissue oxygen delivery enabling these slaves to tolerate stifling conditions in the hull of the slave ship , increased lean muscle mass and therefore greater surface area to volume ratio resulting in easier ability to dissipate heat and remain cool , and increased skin thickness and sebum production resisting the macerating effect of lying in admixed bodily fluids below deck .
	manualset3
107080	11	401848	13	NULL	NULL	0	NULL	anabolic effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that the ability to have survived the middle passage was positively correlated with greater responsiveness of the androgen receptor to its primary ligands dihydrotestosterone and testosterone , and that slaves possessing more responsive androgen receptors experienced a survival advantage engendered by the enhanced anabolic effects which accrued such as increased red cell mass and therefore greater oxygen carrying capacity and tissue oxygen delivery enabling these slaves to tolerate stifling conditions in the hull of the slave ship , increased lean muscle mass and therefore greater surface area to volume ratio resulting in easier ability to dissipate heat and remain cool , and increased skin thickness and sebum production resisting the macerating effect of lying in admixed bodily fluids below deck .
	manualset3
107084	12	401848	13	NULL	NULL	0	NULL	red cell mass	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that the ability to have survived the middle passage was positively correlated with greater responsiveness of the androgen receptor to its primary ligands dihydrotestosterone and testosterone , and that slaves possessing more responsive androgen receptors experienced a survival advantage engendered by the enhanced anabolic effects which accrued such as increased red cell mass and therefore greater oxygen carrying capacity and tissue oxygen delivery enabling these slaves to tolerate stifling conditions in the hull of the slave ship , increased lean muscle mass and therefore greater surface area to volume ratio resulting in easier ability to dissipate heat and remain cool , and increased skin thickness and sebum production resisting the macerating effect of lying in admixed bodily fluids below deck .
	manualset3
107085	13	401848	13	NULL	NULL	0	NULL	greater oxygen carrying capacity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that the ability to have survived the middle passage was positively correlated with greater responsiveness of the androgen receptor to its primary ligands dihydrotestosterone and testosterone , and that slaves possessing more responsive androgen receptors experienced a survival advantage engendered by the enhanced anabolic effects which accrued such as increased red cell mass and therefore greater oxygen carrying capacity and tissue oxygen delivery enabling these slaves to tolerate stifling conditions in the hull of the slave ship , increased lean muscle mass and therefore greater surface area to volume ratio resulting in easier ability to dissipate heat and remain cool , and increased skin thickness and sebum production resisting the macerating effect of lying in admixed bodily fluids below deck .
	manualset3
107086	14	401848	13	NULL	NULL	0	NULL	tissue oxygen delivery	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that the ability to have survived the middle passage was positively correlated with greater responsiveness of the androgen receptor to its primary ligands dihydrotestosterone and testosterone , and that slaves possessing more responsive androgen receptors experienced a survival advantage engendered by the enhanced anabolic effects which accrued such as increased red cell mass and therefore greater oxygen carrying capacity and tissue oxygen delivery enabling these slaves to tolerate stifling conditions in the hull of the slave ship , increased lean muscle mass and therefore greater surface area to volume ratio resulting in easier ability to dissipate heat and remain cool , and increased skin thickness and sebum production resisting the macerating effect of lying in admixed bodily fluids below deck .
	manualset3
107087	15	401848	13	NULL	NULL	0	NULL	slaves	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that the ability to have survived the middle passage was positively correlated with greater responsiveness of the androgen receptor to its primary ligands dihydrotestosterone and testosterone , and that slaves possessing more responsive androgen receptors experienced a survival advantage engendered by the enhanced anabolic effects which accrued such as increased red cell mass and therefore greater oxygen carrying capacity and tissue oxygen delivery enabling these slaves to tolerate stifling conditions in the hull of the slave ship , increased lean muscle mass and therefore greater surface area to volume ratio resulting in easier ability to dissipate heat and remain cool , and increased skin thickness and sebum production resisting the macerating effect of lying in admixed bodily fluids below deck .
	manualset3
107088	16	401848	13	NULL	NULL	0	NULL	conditions 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that the ability to have survived the middle passage was positively correlated with greater responsiveness of the androgen receptor to its primary ligands dihydrotestosterone and testosterone , and that slaves possessing more responsive androgen receptors experienced a survival advantage engendered by the enhanced anabolic effects which accrued such as increased red cell mass and therefore greater oxygen carrying capacity and tissue oxygen delivery enabling these slaves to tolerate stifling conditions in the hull of the slave ship , increased lean muscle mass and therefore greater surface area to volume ratio resulting in easier ability to dissipate heat and remain cool , and increased skin thickness and sebum production resisting the macerating effect of lying in admixed bodily fluids below deck .
	manualset3
107089	17	401848	13	NULL	NULL	0	NULL	hull	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that the ability to have survived the middle passage was positively correlated with greater responsiveness of the androgen receptor to its primary ligands dihydrotestosterone and testosterone , and that slaves possessing more responsive androgen receptors experienced a survival advantage engendered by the enhanced anabolic effects which accrued such as increased red cell mass and therefore greater oxygen carrying capacity and tissue oxygen delivery enabling these slaves to tolerate stifling conditions in the hull of the slave ship , increased lean muscle mass and therefore greater surface area to volume ratio resulting in easier ability to dissipate heat and remain cool , and increased skin thickness and sebum production resisting the macerating effect of lying in admixed bodily fluids below deck .
	manualset3
107090	18	401848	13	NULL	NULL	0	NULL	slave ship	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that the ability to have survived the middle passage was positively correlated with greater responsiveness of the androgen receptor to its primary ligands dihydrotestosterone and testosterone , and that slaves possessing more responsive androgen receptors experienced a survival advantage engendered by the enhanced anabolic effects which accrued such as increased red cell mass and therefore greater oxygen carrying capacity and tissue oxygen delivery enabling these slaves to tolerate stifling conditions in the hull of the slave ship , increased lean muscle mass and therefore greater surface area to volume ratio resulting in easier ability to dissipate heat and remain cool , and increased skin thickness and sebum production resisting the macerating effect of lying in admixed bodily fluids below deck .
	manualset3
107091	19	401848	13	NULL	NULL	0	NULL	lean muscle mass 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that the ability to have survived the middle passage was positively correlated with greater responsiveness of the androgen receptor to its primary ligands dihydrotestosterone and testosterone , and that slaves possessing more responsive androgen receptors experienced a survival advantage engendered by the enhanced anabolic effects which accrued such as increased red cell mass and therefore greater oxygen carrying capacity and tissue oxygen delivery enabling these slaves to tolerate stifling conditions in the hull of the slave ship , increased lean muscle mass and therefore greater surface area to volume ratio resulting in easier ability to dissipate heat and remain cool , and increased skin thickness and sebum production resisting the macerating effect of lying in admixed bodily fluids below deck .
	manualset3
107097	20	401848	13	NULL	NULL	0	NULL	greater surface area to volume ratio 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that the ability to have survived the middle passage was positively correlated with greater responsiveness of the androgen receptor to its primary ligands dihydrotestosterone and testosterone , and that slaves possessing more responsive androgen receptors experienced a survival advantage engendered by the enhanced anabolic effects which accrued such as increased red cell mass and therefore greater oxygen carrying capacity and tissue oxygen delivery enabling these slaves to tolerate stifling conditions in the hull of the slave ship , increased lean muscle mass and therefore greater surface area to volume ratio resulting in easier ability to dissipate heat and remain cool , and increased skin thickness and sebum production resisting the macerating effect of lying in admixed bodily fluids below deck .
	manualset3
107098	21	401848	13	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that the ability to have survived the middle passage was positively correlated with greater responsiveness of the androgen receptor to its primary ligands dihydrotestosterone and testosterone , and that slaves possessing more responsive androgen receptors experienced a survival advantage engendered by the enhanced anabolic effects which accrued such as increased red cell mass and therefore greater oxygen carrying capacity and tissue oxygen delivery enabling these slaves to tolerate stifling conditions in the hull of the slave ship , increased lean muscle mass and therefore greater surface area to volume ratio resulting in easier ability to dissipate heat and remain cool , and increased skin thickness and sebum production resisting the macerating effect of lying in admixed bodily fluids below deck .
	manualset3
107101	24	401848	13	NULL	NULL	0	NULL	skin thickness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that the ability to have survived the middle passage was positively correlated with greater responsiveness of the androgen receptor to its primary ligands dihydrotestosterone and testosterone , and that slaves possessing more responsive androgen receptors experienced a survival advantage engendered by the enhanced anabolic effects which accrued such as increased red cell mass and therefore greater oxygen carrying capacity and tissue oxygen delivery enabling these slaves to tolerate stifling conditions in the hull of the slave ship , increased lean muscle mass and therefore greater surface area to volume ratio resulting in easier ability to dissipate heat and remain cool , and increased skin thickness and sebum production resisting the macerating effect of lying in admixed bodily fluids below deck .
	manualset3
107102	25	401848	13	NULL	NULL	0	NULL	sebum production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that the ability to have survived the middle passage was positively correlated with greater responsiveness of the androgen receptor to its primary ligands dihydrotestosterone and testosterone , and that slaves possessing more responsive androgen receptors experienced a survival advantage engendered by the enhanced anabolic effects which accrued such as increased red cell mass and therefore greater oxygen carrying capacity and tissue oxygen delivery enabling these slaves to tolerate stifling conditions in the hull of the slave ship , increased lean muscle mass and therefore greater surface area to volume ratio resulting in easier ability to dissipate heat and remain cool , and increased skin thickness and sebum production resisting the macerating effect of lying in admixed bodily fluids below deck .
	manualset3
107103	26	401848	13	NULL	NULL	0	NULL	effect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that the ability to have survived the middle passage was positively correlated with greater responsiveness of the androgen receptor to its primary ligands dihydrotestosterone and testosterone , and that slaves possessing more responsive androgen receptors experienced a survival advantage engendered by the enhanced anabolic effects which accrued such as increased red cell mass and therefore greater oxygen carrying capacity and tissue oxygen delivery enabling these slaves to tolerate stifling conditions in the hull of the slave ship , increased lean muscle mass and therefore greater surface area to volume ratio resulting in easier ability to dissipate heat and remain cool , and increased skin thickness and sebum production resisting the macerating effect of lying in admixed bodily fluids below deck .
	manualset3
107104	27	401848	13	NULL	NULL	0	NULL	bodily fluids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that the ability to have survived the middle passage was positively correlated with greater responsiveness of the androgen receptor to its primary ligands dihydrotestosterone and testosterone , and that slaves possessing more responsive androgen receptors experienced a survival advantage engendered by the enhanced anabolic effects which accrued such as increased red cell mass and therefore greater oxygen carrying capacity and tissue oxygen delivery enabling these slaves to tolerate stifling conditions in the hull of the slave ship , increased lean muscle mass and therefore greater surface area to volume ratio resulting in easier ability to dissipate heat and remain cool , and increased skin thickness and sebum production resisting the macerating effect of lying in admixed bodily fluids below deck .
	manualset3
107105	28	401848	13	NULL	NULL	0	NULL	deck	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that the ability to have survived the middle passage was positively correlated with greater responsiveness of the androgen receptor to its primary ligands dihydrotestosterone and testosterone , and that slaves possessing more responsive androgen receptors experienced a survival advantage engendered by the enhanced anabolic effects which accrued such as increased red cell mass and therefore greater oxygen carrying capacity and tissue oxygen delivery enabling these slaves to tolerate stifling conditions in the hull of the slave ship , increased lean muscle mass and therefore greater surface area to volume ratio resulting in easier ability to dissipate heat and remain cool , and increased skin thickness and sebum production resisting the macerating effect of lying in admixed bodily fluids below deck .
	manualset3
107108	1	401849	13	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that these findings might be related to the neurite formation of the senile plaques and to the synaptic involvement in Alzheimer 's disease .
	manualset3
107109	2	401849	13	NULL	NULL	0	NULL	neurite formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that these findings might be related to the neurite formation of the senile plaques and to the synaptic involvement in Alzheimer 's disease .
	manualset3
107110	3	401849	13	NULL	NULL	0	NULL	senile plaques	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that these findings might be related to the neurite formation of the senile plaques and to the synaptic involvement in Alzheimer 's disease .
	manualset3
107111	4	401849	13	NULL	NULL	0	NULL	synaptic involvement 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that these findings might be related to the neurite formation of the senile plaques and to the synaptic involvement in Alzheimer 's disease .
	manualset3
107112	5	401849	13	NULL	NULL	0	NULL	Alzheimer 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It is postulated that these findings might be related to the neurite formation of the senile plaques and to the synaptic involvement in Alzheimer 's disease .
	manualset3
107113	1	401850	13	NULL	NULL	0	NULL	 time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	It is presently the right time for clarifying human papillomavirus ( HPV ) - associated cellular immunity and clinical implications before global HPV vaccination programs begin .
	manualset3
107114	2	401850	13	NULL	NULL	0	NULL	human papillomavirus ( HPV ) - associated cellular immunity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is presently the right time for clarifying human papillomavirus ( HPV ) - associated cellular immunity and clinical implications before global HPV vaccination programs begin .
	manualset3
107115	3	401850	13	NULL	NULL	0	NULL	clinical implications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is presently the right time for clarifying human papillomavirus ( HPV ) - associated cellular immunity and clinical implications before global HPV vaccination programs begin .
	manualset3
107116	4	401850	13	NULL	NULL	0	NULL	global HPV vaccination programs	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is presently the right time for clarifying human papillomavirus ( HPV ) - associated cellular immunity and clinical implications before global HPV vaccination programs begin .
	manualset3
107117	1	401851	13	NULL	NULL	0	NULL	saturation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is proposed , that the saturation of the aromatic hydroxylation , catalyzed by a high affinity site or subspecies of cytochrome P-450 with a low capacity , contributes to the dose-dependent kinetics in vivo .
	manualset3
107119	2	401851	13	NULL	NULL	0	NULL	aromatic hydroxylation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is proposed , that the saturation of the aromatic hydroxylation , catalyzed by a high affinity site or subspecies of cytochrome P-450 with a low capacity , contributes to the dose-dependent kinetics in vivo .
	manualset3
107123	3	401851	13	NULL	NULL	0	NULL	high affinity site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is proposed , that the saturation of the aromatic hydroxylation , catalyzed by a high affinity site or subspecies of cytochrome P-450 with a low capacity , contributes to the dose-dependent kinetics in vivo .
	manualset3
107125	4	401851	13	NULL	NULL	0	NULL	subspecies of cytochrome P-450 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is proposed , that the saturation of the aromatic hydroxylation , catalyzed by a high affinity site or subspecies of cytochrome P-450 with a low capacity , contributes to the dose-dependent kinetics in vivo .
	manualset3
107126	5	401851	13	NULL	NULL	0	NULL	capacity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is proposed , that the saturation of the aromatic hydroxylation , catalyzed by a high affinity site or subspecies of cytochrome P-450 with a low capacity , contributes to the dose-dependent kinetics in vivo .
	manualset3
107127	6	401851	13	NULL	NULL	0	NULL	 dose-dependent kinetics	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is proposed , that the saturation of the aromatic hydroxylation , catalyzed by a high affinity site or subspecies of cytochrome P-450 with a low capacity , contributes to the dose-dependent kinetics in vivo .
	manualset3
107128	1	401852	13	NULL	NULL	0	NULL	pool of glutathione	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	It is proposed that an adequate pool of glutathione is essential to prevent this increase in sulfhdryl oxidation .
	manualset3
107129	2	401852	13	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is proposed that an adequate pool of glutathione is essential to prevent this increase in sulfhdryl oxidation .
	manualset3
107130	3	401852	13	NULL	NULL	0	NULL	sulfhdryl oxidation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is proposed that an adequate pool of glutathione is essential to prevent this increase in sulfhdryl oxidation .
	manualset3
107131	1	401853	13	NULL	NULL	0	NULL	temperature-dependent enzyme ( s )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is proposed that certain temperature-dependent enzyme ( s ) associated with DNA replication kinetics may be involved in the formation of SCEs .
	manualset3
107132	2	401853	13	NULL	NULL	0	NULL	DNA replication kinetics	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is proposed that certain temperature-dependent enzyme ( s ) associated with DNA replication kinetics may be involved in the formation of SCEs .
	manualset3
107133	3	401853	13	NULL	NULL	0	NULL	formation of SCEs	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is proposed that certain temperature-dependent enzyme ( s ) associated with DNA replication kinetics may be involved in the formation of SCEs .
	manualset3
107134	1	401854	13	NULL	NULL	0	NULL	electron attachment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is proposed that electron attachment at very low energy proceeds via dipole bound states , supported by the large dipole moment of the molecule ( 6.2 D ) .
	manualset3
107136	2	401854	13	NULL	NULL	0	NULL	energy	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is proposed that electron attachment at very low energy proceeds via dipole bound states , supported by the large dipole moment of the molecule ( 6.2 D ) .
	manualset3
107138	3	401854	13	NULL	NULL	0	NULL	states	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is proposed that electron attachment at very low energy proceeds via dipole bound states , supported by the large dipole moment of the molecule ( 6.2 D ) .
	manualset3
107141	4	401854	13	NULL	NULL	0	NULL	 dipole moment	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is proposed that electron attachment at very low energy proceeds via dipole bound states , supported by the large dipole moment of the molecule ( 6.2 D ) .
	manualset3
107142	5	401854	13	NULL	NULL	0	NULL	molecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	It is proposed that electron attachment at very low energy proceeds via dipole bound states , supported by the large dipole moment of the molecule ( 6.2 D ) .
	manualset3
107144	6	401854	13	NULL	NULL	0	NULL	6.2 D	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is proposed that electron attachment at very low energy proceeds via dipole bound states , supported by the large dipole moment of the molecule ( 6.2 D ) .
	manualset3
107146	1	401855	13	NULL	NULL	0	NULL	group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is proposed that this group may correspond to a variety of AD who , in addition to symptoms of AD , present characteristics of primary progressive aphasia .
	manualset3
107147	2	401855	13	NULL	NULL	0	NULL	variety of AD 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It is proposed that this group may correspond to a variety of AD who , in addition to symptoms of AD , present characteristics of primary progressive aphasia .
	manualset3
107148	3	401855	13	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is proposed that this group may correspond to a variety of AD who , in addition to symptoms of AD , present characteristics of primary progressive aphasia .
	manualset3
107149	4	401855	13	NULL	NULL	0	NULL	symptoms of AD	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is proposed that this group may correspond to a variety of AD who , in addition to symptoms of AD , present characteristics of primary progressive aphasia .
	manualset3
107150	5	401855	13	NULL	NULL	0	NULL	 characteristics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is proposed that this group may correspond to a variety of AD who , in addition to symptoms of AD , present characteristics of primary progressive aphasia .
	manualset3
107151	6	401855	13	NULL	NULL	0	NULL	primary progressive aphasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is proposed that this group may correspond to a variety of AD who , in addition to symptoms of AD , present characteristics of primary progressive aphasia .
	manualset3
107152	1	401856	13	NULL	NULL	0	NULL	symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is rarely diagnosed and less likely to cause any symptoms during infancy , but approximately more than half become symptomatic around their fifth decade .
	manualset3
107153	2	401856	13	NULL	NULL	0	NULL	infancy	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	It is rarely diagnosed and less likely to cause any symptoms during infancy , but approximately more than half become symptomatic around their fifth decade .
	manualset3
107154	3	401856	13	NULL	NULL	0	NULL	approximately more than half 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is rarely diagnosed and less likely to cause any symptoms during infancy , but approximately more than half become symptomatic around their fifth decade .
	manualset3
107155	4	401856	13	NULL	NULL	0	NULL	fifth decade	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	It is rarely diagnosed and less likely to cause any symptoms during infancy , but approximately more than half become symptomatic around their fifth decade .
	manualset3
107156	1	401857	13	NULL	NULL	0	NULL	IABP	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is reasonable to initiate IABP and hemofiltration dialysis during the early stages for the appropriate control of hemodynamics and fluid in shock patients with cardiac amyloidosis .
	manualset3
107157	2	401857	13	NULL	NULL	0	NULL	hemofiltration dialysis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is reasonable to initiate IABP and hemofiltration dialysis during the early stages for the appropriate control of hemodynamics and fluid in shock patients with cardiac amyloidosis .
	manualset3
107158	3	401857	13	NULL	NULL	0	NULL	early stages	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	It is reasonable to initiate IABP and hemofiltration dialysis during the early stages for the appropriate control of hemodynamics and fluid in shock patients with cardiac amyloidosis .
	manualset3
107159	4	401857	13	NULL	NULL	0	NULL	control of hemodynamics 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is reasonable to initiate IABP and hemofiltration dialysis during the early stages for the appropriate control of hemodynamics and fluid in shock patients with cardiac amyloidosis .
	manualset3
107160	5	401857	13	NULL	NULL	0	NULL	control of fluid	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is reasonable to initiate IABP and hemofiltration dialysis during the early stages for the appropriate control of hemodynamics and fluid in shock patients with cardiac amyloidosis .
	manualset3
107161	6	401857	13	NULL	NULL	0	NULL	shock patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is reasonable to initiate IABP and hemofiltration dialysis during the early stages for the appropriate control of hemodynamics and fluid in shock patients with cardiac amyloidosis .
	manualset3
107162	7	401857	13	NULL	NULL	0	NULL	 cardiac amyloidosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is reasonable to initiate IABP and hemofiltration dialysis during the early stages for the appropriate control of hemodynamics and fluid in shock patients with cardiac amyloidosis .
	manualset3
107163	1	401858	13	NULL	NULL	0	NULL	7 - and 12-thienylbenz ( a ) anthracenes 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	7 - and 12-thienylbenz ( a ) anthracenes .
	manualset3
107168	1	401859	13	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that , until the association between fibrinolysis and worse outcome is investigated further , patients showing fibrinolysis early after cardiopulmonary bypass should not be discharged too soon from intensive care .
	manualset3
107170	2	401859	13	NULL	NULL	0	NULL	fibrinolysis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that , until the association between fibrinolysis and worse outcome is investigated further , patients showing fibrinolysis early after cardiopulmonary bypass should not be discharged too soon from intensive care .
	manualset3
107172	3	401859	13	NULL	NULL	0	NULL	outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that , until the association between fibrinolysis and worse outcome is investigated further , patients showing fibrinolysis early after cardiopulmonary bypass should not be discharged too soon from intensive care .
	manualset3
107173	4	401859	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that , until the association between fibrinolysis and worse outcome is investigated further , patients showing fibrinolysis early after cardiopulmonary bypass should not be discharged too soon from intensive care .
	manualset3
107175	5	401859	13	NULL	NULL	0	NULL	fibrinolysis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that , until the association between fibrinolysis and worse outcome is investigated further , patients showing fibrinolysis early after cardiopulmonary bypass should not be discharged too soon from intensive care .
	manualset3
107177	6	401859	13	NULL	NULL	0	NULL	cardiopulmonary bypass 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that , until the association between fibrinolysis and worse outcome is investigated further , patients showing fibrinolysis early after cardiopulmonary bypass should not be discharged too soon from intensive care .
	manualset3
107178	7	401859	13	NULL	NULL	0	NULL	 intensive care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that , until the association between fibrinolysis and worse outcome is investigated further , patients showing fibrinolysis early after cardiopulmonary bypass should not be discharged too soon from intensive care .
	manualset3
107183	1	401860	13	NULL	NULL	0	NULL	infusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that a routine infusion of lidocaine , 100 mg bolus followed by 2 mg.kg-1 , be given to every postoperative coronary artery bypass patient for at least the first 24 hours .
	manualset3
107185	2	401860	13	NULL	NULL	0	NULL	lidocaine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that a routine infusion of lidocaine , 100 mg bolus followed by 2 mg.kg-1 , be given to every postoperative coronary artery bypass patient for at least the first 24 hours .
	manualset3
107186	3	401860	13	NULL	NULL	0	NULL	100 mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that a routine infusion of lidocaine , 100 mg bolus followed by 2 mg.kg-1 , be given to every postoperative coronary artery bypass patient for at least the first 24 hours .
	manualset3
107187	4	401860	13	NULL	NULL	0	NULL	2 mg.kg-1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that a routine infusion of lidocaine , 100 mg bolus followed by 2 mg.kg-1 , be given to every postoperative coronary artery bypass patient for at least the first 24 hours .
	manualset3
107190	5	401860	13	NULL	NULL	0	NULL	postoperative coronary artery bypass patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that a routine infusion of lidocaine , 100 mg bolus followed by 2 mg.kg-1 , be given to every postoperative coronary artery bypass patient for at least the first 24 hours .
	manualset3
107192	6	401860	13	NULL	NULL	0	NULL	first 24 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that a routine infusion of lidocaine , 100 mg bolus followed by 2 mg.kg-1 , be given to every postoperative coronary artery bypass patient for at least the first 24 hours .
	manualset3
107195	1	401861	13	NULL	NULL	0	NULL	 investigative data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that all investigative and autopsy data be considered and that the cause of death not be certified based purely on blood HCQ concentrations .
	manualset3
107196	2	401861	13	NULL	NULL	0	NULL	autopsy data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that all investigative and autopsy data be considered and that the cause of death not be certified based purely on blood HCQ concentrations .
	manualset3
107197	3	401861	13	NULL	NULL	0	NULL	cause of death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that all investigative and autopsy data be considered and that the cause of death not be certified based purely on blood HCQ concentrations .
	manualset3
107198	4	401861	13	NULL	NULL	0	NULL	blood HCQ concentrations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that all investigative and autopsy data be considered and that the cause of death not be certified based purely on blood HCQ concentrations .
	manualset3
107207	1	401862	13	NULL	NULL	0	NULL	 expansion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that expansion of PCA programs with abdominal surgery patients be considered only in cases where there is fiscal advantage or where patient satisfaction can be a driving force .
	manualset3
107209	2	401862	13	NULL	NULL	0	NULL	PCA programs	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that expansion of PCA programs with abdominal surgery patients be considered only in cases where there is fiscal advantage or where patient satisfaction can be a driving force .
	manualset3
107211	3	401862	13	NULL	NULL	0	NULL	abdominal surgery patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that expansion of PCA programs with abdominal surgery patients be considered only in cases where there is fiscal advantage or where patient satisfaction can be a driving force .
	manualset3
107213	4	401862	13	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that expansion of PCA programs with abdominal surgery patients be considered only in cases where there is fiscal advantage or where patient satisfaction can be a driving force .
	manualset3
107216	5	401862	13	NULL	NULL	0	NULL	fiscal advantage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that expansion of PCA programs with abdominal surgery patients be considered only in cases where there is fiscal advantage or where patient satisfaction can be a driving force .
	manualset3
107218	6	401862	13	NULL	NULL	0	NULL	patient satisfaction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that expansion of PCA programs with abdominal surgery patients be considered only in cases where there is fiscal advantage or where patient satisfaction can be a driving force .
	manualset3
107219	7	401862	13	NULL	NULL	0	NULL	force	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that expansion of PCA programs with abdominal surgery patients be considered only in cases where there is fiscal advantage or where patient satisfaction can be a driving force .
	manualset3
107248	1	401863	13	NULL	NULL	0	NULL	countries	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that in countries where sheep breeding is aseasonal a sexual rest of infected ewes for at least 4 months must be part of any program for the control and eradication of ram epididymitis .
	manualset3
107249	2	401863	13	NULL	NULL	0	NULL	sheep	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that in countries where sheep breeding is aseasonal a sexual rest of infected ewes for at least 4 months must be part of any program for the control and eradication of ram epididymitis .
	manualset3
107250	3	401863	13	NULL	NULL	0	NULL	sexual rest	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that in countries where sheep breeding is aseasonal a sexual rest of infected ewes for at least 4 months must be part of any program for the control and eradication of ram epididymitis .
	manualset3
107251	4	401863	13	NULL	NULL	0	NULL	ewes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that in countries where sheep breeding is aseasonal a sexual rest of infected ewes for at least 4 months must be part of any program for the control and eradication of ram epididymitis .
	manualset3
107252	5	401863	13	NULL	NULL	0	NULL	4 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that in countries where sheep breeding is aseasonal a sexual rest of infected ewes for at least 4 months must be part of any program for the control and eradication of ram epididymitis .
	manualset3
107253	6	401863	13	NULL	NULL	0	NULL	part of any program 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that in countries where sheep breeding is aseasonal a sexual rest of infected ewes for at least 4 months must be part of any program for the control and eradication of ram epididymitis .
	manualset3
107254	7	401863	13	NULL	NULL	0	NULL	control 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that in countries where sheep breeding is aseasonal a sexual rest of infected ewes for at least 4 months must be part of any program for the control and eradication of ram epididymitis .
	manualset3
107256	8	401863	13	NULL	NULL	0	NULL	eradication 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that in countries where sheep breeding is aseasonal a sexual rest of infected ewes for at least 4 months must be part of any program for the control and eradication of ram epididymitis .
	manualset3
107257	9	401863	13	NULL	NULL	0	NULL	 ram epididymitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that in countries where sheep breeding is aseasonal a sexual rest of infected ewes for at least 4 months must be part of any program for the control and eradication of ram epididymitis .
	manualset3
107258	1	401864	13	NULL	NULL	0	NULL	chylomicrons	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that when chylomicrons are present they be removed prior to diagnostic and quantitative lipoprotein electrophoresis in agarose gel .
	manualset3
107259	2	401864	13	NULL	NULL	0	NULL	quantitative lipoprotein electrophoresis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that when chylomicrons are present they be removed prior to diagnostic and quantitative lipoprotein electrophoresis in agarose gel .
	manualset3
107260	3	401864	13	NULL	NULL	0	NULL	agarose gel	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that when chylomicrons are present they be removed prior to diagnostic and quantitative lipoprotein electrophoresis in agarose gel .
	manualset3
108306	4	401864	13	NULL	NULL	0	NULL	diagnostic lipoprotein electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	It is recommended that when chylomicrons are present they be removed prior to diagnostic and quantitative lipoprotein electrophoresis in agarose gel .
	manualset3
107261	1	401865	13	NULL	NULL	0	NULL	variety of new tools	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown here that a variety of new tools and methods based on internal standard technology are now being developed to code globally all peptides in control and experimental samples for quantification .
	manualset3
107262	2	401865	13	NULL	NULL	0	NULL	methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown here that a variety of new tools and methods based on internal standard technology are now being developed to code globally all peptides in control and experimental samples for quantification .
	manualset3
107263	3	401865	13	NULL	NULL	0	NULL	internal standard technology 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown here that a variety of new tools and methods based on internal standard technology are now being developed to code globally all peptides in control and experimental samples for quantification .
	manualset3
107265	4	401865	13	NULL	NULL	0	NULL	peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown here that a variety of new tools and methods based on internal standard technology are now being developed to code globally all peptides in control and experimental samples for quantification .
	manualset3
107270	5	401865	13	NULL	NULL	0	NULL	control samples	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown here that a variety of new tools and methods based on internal standard technology are now being developed to code globally all peptides in control and experimental samples for quantification .
	manualset3
107273	6	401865	13	NULL	NULL	0	NULL	experimental samples	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown here that a variety of new tools and methods based on internal standard technology are now being developed to code globally all peptides in control and experimental samples for quantification .
	manualset3
107275	7	401865	13	NULL	NULL	0	NULL	quantification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown here that a variety of new tools and methods based on internal standard technology are now being developed to code globally all peptides in control and experimental samples for quantification .
	manualset3
107683	1	401866	13	NULL	NULL	0	NULL	aging changes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that aging changes substantially influence proliferative activity of the PDL cells and subsequent tooth movement during the initial phase in particular .
	manualset3
107684	2	401866	13	NULL	NULL	0	NULL	 proliferative activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that aging changes substantially influence proliferative activity of the PDL cells and subsequent tooth movement during the initial phase in particular .
	manualset3
107685	3	401866	13	NULL	NULL	0	NULL	PDL cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that aging changes substantially influence proliferative activity of the PDL cells and subsequent tooth movement during the initial phase in particular .
	manualset3
107686	4	401866	13	NULL	NULL	0	NULL	subsequent tooth movement 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that aging changes substantially influence proliferative activity of the PDL cells and subsequent tooth movement during the initial phase in particular .
	manualset3
107687	5	401866	13	NULL	NULL	0	NULL	initial phase	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that aging changes substantially influence proliferative activity of the PDL cells and subsequent tooth movement during the initial phase in particular .
	manualset3
107688	1	401867	13	NULL	NULL	0	NULL	 bicellar nematic liquid-crystalline phases	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that bicellar nematic liquid-crystalline phases can be oriented with the director ( the normal to the bicellar plane ) at an arbitrary angle to the applied magnetic field by sample rotation around one axis ( variable-angle sample spinning ) or around two axes successively ( switched-angle spinning ) .
	manualset3
107689	2	401867	13	NULL	NULL	0	NULL	director	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that bicellar nematic liquid-crystalline phases can be oriented with the director ( the normal to the bicellar plane ) at an arbitrary angle to the applied magnetic field by sample rotation around one axis ( variable-angle sample spinning ) or around two axes successively ( switched-angle spinning ) .
	manualset3
107690	3	401867	13	NULL	NULL	0	NULL	bicellar plane	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that bicellar nematic liquid-crystalline phases can be oriented with the director ( the normal to the bicellar plane ) at an arbitrary angle to the applied magnetic field by sample rotation around one axis ( variable-angle sample spinning ) or around two axes successively ( switched-angle spinning ) .
	manualset3
107691	4	401867	13	NULL	NULL	0	NULL	arbitrary angle	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that bicellar nematic liquid-crystalline phases can be oriented with the director ( the normal to the bicellar plane ) at an arbitrary angle to the applied magnetic field by sample rotation around one axis ( variable-angle sample spinning ) or around two axes successively ( switched-angle spinning ) .
	manualset3
107692	5	401867	13	NULL	NULL	0	NULL	magnetic field	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that bicellar nematic liquid-crystalline phases can be oriented with the director ( the normal to the bicellar plane ) at an arbitrary angle to the applied magnetic field by sample rotation around one axis ( variable-angle sample spinning ) or around two axes successively ( switched-angle spinning ) .
	manualset3
107693	6	401867	13	NULL	NULL	0	NULL	sample rotation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that bicellar nematic liquid-crystalline phases can be oriented with the director ( the normal to the bicellar plane ) at an arbitrary angle to the applied magnetic field by sample rotation around one axis ( variable-angle sample spinning ) or around two axes successively ( switched-angle spinning ) .
	manualset3
107694	7	401867	13	NULL	NULL	0	NULL	axis 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that bicellar nematic liquid-crystalline phases can be oriented with the director ( the normal to the bicellar plane ) at an arbitrary angle to the applied magnetic field by sample rotation around one axis ( variable-angle sample spinning ) or around two axes successively ( switched-angle spinning ) .
	manualset3
107695	8	401867	13	NULL	NULL	NULL	NULL	 variable-angle	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is shown that bicellar nematic liquid-crystalline phases can be oriented with the director ( the normal to the bicellar plane ) at an arbitrary angle to the applied magnetic field by sample rotation around one axis ( variable-angle sample spinning ) or around two axes successively ( switched-angle spinning ) .
	manualset3
107696	9	401867	13	NULL	NULL	NULL	NULL	sample spinning 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is shown that bicellar nematic liquid-crystalline phases can be oriented with the director ( the normal to the bicellar plane ) at an arbitrary angle to the applied magnetic field by sample rotation around one axis ( variable-angle sample spinning ) or around two axes successively ( switched-angle spinning ) .
	manualset3
107697	10	401867	13	NULL	NULL	0	NULL	 two axes 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that bicellar nematic liquid-crystalline phases can be oriented with the director ( the normal to the bicellar plane ) at an arbitrary angle to the applied magnetic field by sample rotation around one axis ( variable-angle sample spinning ) or around two axes successively ( switched-angle spinning ) .
	manualset3
107698	11	401867	13	NULL	NULL	0	NULL	switched-angle spinning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that bicellar nematic liquid-crystalline phases can be oriented with the director ( the normal to the bicellar plane ) at an arbitrary angle to the applied magnetic field by sample rotation around one axis ( variable-angle sample spinning ) or around two axes successively ( switched-angle spinning ) .
	manualset3
107699	1	401868	13	NULL	NULL	0	NULL	inverse planning method 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the conventional inverse planning method for optimizing incident intensity can be extended to include a ` concurrent ' leaf sequencing operation from which the leakage and head scatter corrections are determined .
	manualset3
107700	2	401868	13	NULL	NULL	0	NULL	 incident intensity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the conventional inverse planning method for optimizing incident intensity can be extended to include a ` concurrent ' leaf sequencing operation from which the leakage and head scatter corrections are determined .
	manualset3
107701	3	401868	13	NULL	NULL	0	NULL	 include	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the conventional inverse planning method for optimizing incident intensity can be extended to include a ` concurrent ' leaf sequencing operation from which the leakage and head scatter corrections are determined .
	manualset3
107702	4	401868	13	NULL	NULL	0	NULL	leaf sequencing operation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the conventional inverse planning method for optimizing incident intensity can be extended to include a ` concurrent ' leaf sequencing operation from which the leakage and head scatter corrections are determined .
	manualset3
107703	5	401868	13	NULL	NULL	0	NULL	 leakage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the conventional inverse planning method for optimizing incident intensity can be extended to include a ` concurrent ' leaf sequencing operation from which the leakage and head scatter corrections are determined .
	manualset3
107704	6	401868	13	NULL	NULL	0	NULL	head scatter corrections	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the conventional inverse planning method for optimizing incident intensity can be extended to include a ` concurrent ' leaf sequencing operation from which the leakage and head scatter corrections are determined .
	manualset3
107705	1	401869	13	NULL	NULL	0	NULL	distribution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the distribution of carbonic anhydrase II is much similar in all of these acid producing cells : most of the enzyme is cytoplasmic and nucleoplasmic and only a small fraction of the enzyme is associated with the apical plasma membrane .
	manualset3
107706	2	401869	13	NULL	NULL	0	NULL	carbonic anhydrase II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the distribution of carbonic anhydrase II is much similar in all of these acid producing cells : most of the enzyme is cytoplasmic and nucleoplasmic and only a small fraction of the enzyme is associated with the apical plasma membrane .
	manualset3
107707	3	401869	13	NULL	NULL	0	NULL	acid producing cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the distribution of carbonic anhydrase II is much similar in all of these acid producing cells : most of the enzyme is cytoplasmic and nucleoplasmic and only a small fraction of the enzyme is associated with the apical plasma membrane .
	manualset3
107708	4	401869	13	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the distribution of carbonic anhydrase II is much similar in all of these acid producing cells : most of the enzyme is cytoplasmic and nucleoplasmic and only a small fraction of the enzyme is associated with the apical plasma membrane .
	manualset3
107709	5	401869	13	NULL	NULL	0	NULL	small fraction	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the distribution of carbonic anhydrase II is much similar in all of these acid producing cells : most of the enzyme is cytoplasmic and nucleoplasmic and only a small fraction of the enzyme is associated with the apical plasma membrane .
	manualset3
107710	6	401869	13	NULL	NULL	0	NULL	enzyme 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the distribution of carbonic anhydrase II is much similar in all of these acid producing cells : most of the enzyme is cytoplasmic and nucleoplasmic and only a small fraction of the enzyme is associated with the apical plasma membrane .
	manualset3
107711	7	401869	13	NULL	NULL	0	NULL	apical plasma membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the distribution of carbonic anhydrase II is much similar in all of these acid producing cells : most of the enzyme is cytoplasmic and nucleoplasmic and only a small fraction of the enzyme is associated with the apical plasma membrane .
	manualset3
107712	1	401870	13	NULL	NULL	0	NULL	experimental measurements	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the experimental measurements commonly made in biological and synthetic membrane studies may be used , with minor modification , to obtain the phenomenological transport coefficients and their concentration dependences .
	manualset3
107713	2	401870	13	NULL	NULL	0	NULL	biological membrane studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the experimental measurements commonly made in biological and synthetic membrane studies may be used , with minor modification , to obtain the phenomenological transport coefficients and their concentration dependences .
	manualset3
107714	3	401870	13	NULL	NULL	0	NULL	synthetic membrane studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the experimental measurements commonly made in biological and synthetic membrane studies may be used , with minor modification , to obtain the phenomenological transport coefficients and their concentration dependences .
	manualset3
107715	4	401870	13	NULL	NULL	0	NULL	minor modification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the experimental measurements commonly made in biological and synthetic membrane studies may be used , with minor modification , to obtain the phenomenological transport coefficients and their concentration dependences .
	manualset3
107716	5	401870	13	NULL	NULL	0	NULL	transport coefficients	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the experimental measurements commonly made in biological and synthetic membrane studies may be used , with minor modification , to obtain the phenomenological transport coefficients and their concentration dependences .
	manualset3
107717	6	401870	13	NULL	NULL	0	NULL	concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the experimental measurements commonly made in biological and synthetic membrane studies may be used , with minor modification , to obtain the phenomenological transport coefficients and their concentration dependences .
	manualset3
107718	7	401870	13	NULL	NULL	0	NULL	dependences 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the experimental measurements commonly made in biological and synthetic membrane studies may be used , with minor modification , to obtain the phenomenological transport coefficients and their concentration dependences .
	manualset3
107719	1	401871	13	NULL	NULL	0	NULL	flavin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the flavin is not essential for assembly and membrane binding of succinate dehydrogenase in B. subtilis .
	manualset3
107720	2	401871	13	NULL	NULL	NULL	NULL	assembly	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is shown that the flavin is not essential for assembly and membrane binding of succinate dehydrogenase in B. subtilis .
	manualset3
107721	3	401871	13	NULL	NULL	0	NULL	 membrane binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the flavin is not essential for assembly and membrane binding of succinate dehydrogenase in B. subtilis .
	manualset3
107722	4	401871	13	NULL	NULL	0	NULL	succinate dehydrogenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the flavin is not essential for assembly and membrane binding of succinate dehydrogenase in B. subtilis .
	manualset3
107723	5	401871	13	NULL	NULL	0	NULL	B. subtilis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the flavin is not essential for assembly and membrane binding of succinate dehydrogenase in B. subtilis .
	manualset3
107724	1	401872	13	NULL	NULL	0	NULL	70-year-old woman	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	70-year-old woman with chest pain and new diastolic murmur 6 months after coronary artery bypass grafting .
	manualset3
107725	2	401872	13	NULL	NULL	0	NULL	chest pain 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	70-year-old woman with chest pain and new diastolic murmur 6 months after coronary artery bypass grafting .
	manualset3
107726	3	401872	13	NULL	NULL	0	NULL	diastolic murmur	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	70-year-old woman with chest pain and new diastolic murmur 6 months after coronary artery bypass grafting .
	manualset3
107727	4	401872	13	NULL	NULL	0	NULL	6 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	70-year-old woman with chest pain and new diastolic murmur 6 months after coronary artery bypass grafting .
	manualset3
107728	5	401872	13	NULL	NULL	0	NULL	coronary artery bypass grafting	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	70-year-old woman with chest pain and new diastolic murmur 6 months after coronary artery bypass grafting .
	manualset3
107729	1	401873	13	NULL	NULL	0	NULL	models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the models can be extended to account for a composite membrane geometry , by deposition of a thin polysulfone film onto the support .
	manualset3
107730	2	401873	13	NULL	NULL	0	NULL	composite membrane geometry	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the models can be extended to account for a composite membrane geometry , by deposition of a thin polysulfone film onto the support .
	manualset3
107731	3	401873	13	NULL	NULL	0	NULL	 deposition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the models can be extended to account for a composite membrane geometry , by deposition of a thin polysulfone film onto the support .
	manualset3
107732	4	401873	13	NULL	NULL	0	NULL	polysulfone film	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the models can be extended to account for a composite membrane geometry , by deposition of a thin polysulfone film onto the support .
	manualset3
107733	5	401873	13	NULL	NULL	0	NULL	support 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the models can be extended to account for a composite membrane geometry , by deposition of a thin polysulfone film onto the support .
	manualset3
107734	1	401874	13	NULL	NULL	0	NULL	variation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the variation of the tray transmission factor with field size and source-surface distance can easily be taken into account in the dose calculation by considering the volume of the irradiated tray material and the position of the tray in the beam .
	manualset3
107735	2	401874	13	NULL	NULL	0	NULL	tray transmission factor	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the variation of the tray transmission factor with field size and source-surface distance can easily be taken into account in the dose calculation by considering the volume of the irradiated tray material and the position of the tray in the beam .
	manualset3
107736	3	401874	13	NULL	NULL	0	NULL	field size 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the variation of the tray transmission factor with field size and source-surface distance can easily be taken into account in the dose calculation by considering the volume of the irradiated tray material and the position of the tray in the beam .
	manualset3
107737	4	401874	13	NULL	NULL	0	NULL	source-surface distance	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the variation of the tray transmission factor with field size and source-surface distance can easily be taken into account in the dose calculation by considering the volume of the irradiated tray material and the position of the tray in the beam .
	manualset3
107738	5	401874	13	NULL	NULL	0	NULL	 account	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the variation of the tray transmission factor with field size and source-surface distance can easily be taken into account in the dose calculation by considering the volume of the irradiated tray material and the position of the tray in the beam .
	manualset3
107739	6	401874	13	NULL	NULL	0	NULL	dose calculation	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the variation of the tray transmission factor with field size and source-surface distance can easily be taken into account in the dose calculation by considering the volume of the irradiated tray material and the position of the tray in the beam .
	manualset3
107740	7	401874	13	NULL	NULL	0	NULL	volume 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the variation of the tray transmission factor with field size and source-surface distance can easily be taken into account in the dose calculation by considering the volume of the irradiated tray material and the position of the tray in the beam .
	manualset3
107741	8	401874	13	NULL	NULL	0	NULL	 tray material 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the variation of the tray transmission factor with field size and source-surface distance can easily be taken into account in the dose calculation by considering the volume of the irradiated tray material and the position of the tray in the beam .
	manualset3
107742	9	401874	13	NULL	NULL	0	NULL	position of the tray 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the variation of the tray transmission factor with field size and source-surface distance can easily be taken into account in the dose calculation by considering the volume of the irradiated tray material and the position of the tray in the beam .
	manualset3
107743	10	401874	13	NULL	NULL	0	NULL	beam	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the variation of the tray transmission factor with field size and source-surface distance can easily be taken into account in the dose calculation by considering the volume of the irradiated tray material and the position of the tray in the beam .
	manualset3
107744	1	401875	13	NULL	NULL	0	NULL	cone	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that these are minimized by moving cone and detector in a nearly theta-2theta motion and by using a small-angle sector .
	manualset3
107745	2	401875	13	NULL	NULL	0	NULL	detector 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that these are minimized by moving cone and detector in a nearly theta-2theta motion and by using a small-angle sector .
	manualset3
107746	3	401875	13	NULL	NULL	0	NULL	theta-2theta motion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that these are minimized by moving cone and detector in a nearly theta-2theta motion and by using a small-angle sector .
	manualset3
107747	4	401875	13	NULL	NULL	0	NULL	small-angle sector	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that these are minimized by moving cone and detector in a nearly theta-2theta motion and by using a small-angle sector .
	manualset3
107748	1	401876	13	NULL	NULL	0	NULL	conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that under certain limiting conditions the apparent allosteric interaction between ligands is equal to the conformational interaction between subunits .
	manualset3
107749	2	401876	13	NULL	NULL	0	NULL	allosteric interaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that under certain limiting conditions the apparent allosteric interaction between ligands is equal to the conformational interaction between subunits .
	manualset3
107750	3	401876	13	NULL	NULL	0	NULL	ligands	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that under certain limiting conditions the apparent allosteric interaction between ligands is equal to the conformational interaction between subunits .
	manualset3
107751	4	401876	13	NULL	NULL	0	NULL	conformational interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that under certain limiting conditions the apparent allosteric interaction between ligands is equal to the conformational interaction between subunits .
	manualset3
107752	5	401876	13	NULL	NULL	0	NULL	subunits	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that under certain limiting conditions the apparent allosteric interaction between ligands is equal to the conformational interaction between subunits .
	manualset3
107753	1	401877	13	NULL	NULL	0	NULL	 treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is similarly not known whether treatment with sulphonylurea , metformin or insulin is particularly beneficial or whether any of these therapies is potentially harmful .
	manualset3
107754	2	401877	13	NULL	NULL	0	NULL	 sulphonylurea	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	It is similarly not known whether treatment with sulphonylurea , metformin or insulin is particularly beneficial or whether any of these therapies is potentially harmful .
	manualset3
107755	3	401877	13	NULL	NULL	0	NULL	metformin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	It is similarly not known whether treatment with sulphonylurea , metformin or insulin is particularly beneficial or whether any of these therapies is potentially harmful .
	manualset3
107756	4	401877	13	NULL	NULL	0	NULL	insulin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	It is similarly not known whether treatment with sulphonylurea , metformin or insulin is particularly beneficial or whether any of these therapies is potentially harmful .
	manualset3
107757	5	401877	13	NULL	NULL	0	NULL	therapies 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is similarly not known whether treatment with sulphonylurea , metformin or insulin is particularly beneficial or whether any of these therapies is potentially harmful .
	manualset3
107758	1	401878	13	NULL	NULL	0	NULL	complications 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is sometimes accompanied by complications such as alveolar osteitis , secondary infection , hemorrhage , dysesthesia and , most severely , iatrogenic fracture .
	manualset3
107759	2	401878	13	NULL	NULL	0	NULL	alveolar osteitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is sometimes accompanied by complications such as alveolar osteitis , secondary infection , hemorrhage , dysesthesia and , most severely , iatrogenic fracture .
	manualset3
107760	3	401878	13	NULL	NULL	0	NULL	secondary infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is sometimes accompanied by complications such as alveolar osteitis , secondary infection , hemorrhage , dysesthesia and , most severely , iatrogenic fracture .
	manualset3
107761	4	401878	13	NULL	NULL	0	NULL	hemorrhage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is sometimes accompanied by complications such as alveolar osteitis , secondary infection , hemorrhage , dysesthesia and , most severely , iatrogenic fracture .
	manualset3
107762	5	401878	13	NULL	NULL	0	NULL	dysesthesia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is sometimes accompanied by complications such as alveolar osteitis , secondary infection , hemorrhage , dysesthesia and , most severely , iatrogenic fracture .
	manualset3
107763	6	401878	13	NULL	NULL	0	NULL	iatrogenic fracture	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is sometimes accompanied by complications such as alveolar osteitis , secondary infection , hemorrhage , dysesthesia and , most severely , iatrogenic fracture .
	manualset3
107764	1	401879	13	NULL	NULL	0	NULL	NGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested here that NGF and other growth factors may have a role in the evolution and development of the uniquely human capacity to produce emotional tears .
	manualset3
107765	2	401879	13	NULL	NULL	0	NULL	 growth factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested here that NGF and other growth factors may have a role in the evolution and development of the uniquely human capacity to produce emotional tears .
	manualset3
107766	3	401879	13	NULL	NULL	NULL	NULL	role 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is suggested here that NGF and other growth factors may have a role in the evolution and development of the uniquely human capacity to produce emotional tears .
	manualset3
107767	4	401879	13	NULL	NULL	NULL	NULL	evolution	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is suggested here that NGF and other growth factors may have a role in the evolution and development of the uniquely human capacity to produce emotional tears .
	manualset3
107768	5	401879	13	NULL	NULL	NULL	NULL	development 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is suggested here that NGF and other growth factors may have a role in the evolution and development of the uniquely human capacity to produce emotional tears .
	manualset3
107769	6	401879	13	NULL	NULL	NULL	NULL	human capacity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is suggested here that NGF and other growth factors may have a role in the evolution and development of the uniquely human capacity to produce emotional tears .
	manualset3
107770	7	401879	13	NULL	NULL	0	NULL	emotional tears 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested here that NGF and other growth factors may have a role in the evolution and development of the uniquely human capacity to produce emotional tears .
	manualset3
107771	1	401880	13	NULL	NULL	0	NULL	ATP 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that ATP acts on passive cation movements either by chelation of membrane charge or by a direct interaction with membrane proteins and may be involved in the volume regulation of cation transport in the dog erythrocyte .
	manualset3
107772	2	401880	13	NULL	NULL	0	NULL	acts	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that ATP acts on passive cation movements either by chelation of membrane charge or by a direct interaction with membrane proteins and may be involved in the volume regulation of cation transport in the dog erythrocyte .
	manualset3
107773	3	401880	13	NULL	NULL	0	NULL	passive cation movements 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that ATP acts on passive cation movements either by chelation of membrane charge or by a direct interaction with membrane proteins and may be involved in the volume regulation of cation transport in the dog erythrocyte .
	manualset3
107774	4	401880	13	NULL	NULL	0	NULL	chelation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that ATP acts on passive cation movements either by chelation of membrane charge or by a direct interaction with membrane proteins and may be involved in the volume regulation of cation transport in the dog erythrocyte .
	manualset3
107775	5	401880	13	NULL	NULL	0	NULL	membrane charge	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that ATP acts on passive cation movements either by chelation of membrane charge or by a direct interaction with membrane proteins and may be involved in the volume regulation of cation transport in the dog erythrocyte .
	manualset3
107776	6	401880	13	NULL	NULL	0	NULL	interaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that ATP acts on passive cation movements either by chelation of membrane charge or by a direct interaction with membrane proteins and may be involved in the volume regulation of cation transport in the dog erythrocyte .
	manualset3
107777	7	401880	13	NULL	NULL	0	NULL	membrane proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that ATP acts on passive cation movements either by chelation of membrane charge or by a direct interaction with membrane proteins and may be involved in the volume regulation of cation transport in the dog erythrocyte .
	manualset3
107778	8	401880	13	NULL	NULL	0	NULL	volume regulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that ATP acts on passive cation movements either by chelation of membrane charge or by a direct interaction with membrane proteins and may be involved in the volume regulation of cation transport in the dog erythrocyte .
	manualset3
107779	9	401880	13	NULL	NULL	0	NULL	cation transport	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that ATP acts on passive cation movements either by chelation of membrane charge or by a direct interaction with membrane proteins and may be involved in the volume regulation of cation transport in the dog erythrocyte .
	manualset3
107780	10	401880	13	NULL	NULL	0	NULL	dog erythrocyte	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that ATP acts on passive cation movements either by chelation of membrane charge or by a direct interaction with membrane proteins and may be involved in the volume regulation of cation transport in the dog erythrocyte .
	manualset3
107781	1	401881	13	NULL	NULL	0	NULL	Mo	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that Mo can interfere with the F-poisoning effect and that Mo may well be used as z worth medicine for the prevention and control of this illness .
	manualset3
107782	2	401881	13	NULL	NULL	0	NULL	F-poisoning effect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that Mo can interfere with the F-poisoning effect and that Mo may well be used as z worth medicine for the prevention and control of this illness .
	manualset3
107783	3	401881	13	NULL	NULL	0	NULL	Mo	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that Mo can interfere with the F-poisoning effect and that Mo may well be used as z worth medicine for the prevention and control of this illness .
	manualset3
107784	4	401881	13	NULL	NULL	0	NULL	z worth medicine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that Mo can interfere with the F-poisoning effect and that Mo may well be used as z worth medicine for the prevention and control of this illness .
	manualset3
107785	5	401881	13	NULL	NULL	0	NULL	prevention 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that Mo can interfere with the F-poisoning effect and that Mo may well be used as z worth medicine for the prevention and control of this illness .
	manualset3
107786	6	401881	13	NULL	NULL	0	NULL	control 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that Mo can interfere with the F-poisoning effect and that Mo may well be used as z worth medicine for the prevention and control of this illness .
	manualset3
107787	7	401881	13	NULL	NULL	0	NULL	illness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that Mo can interfere with the F-poisoning effect and that Mo may well be used as z worth medicine for the prevention and control of this illness .
	manualset3
107788	1	401882	13	NULL	NULL	0	NULL	diazotrophic cyanobacterium 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that a diazotrophic cyanobacterium , like Cyanothece sp .
	manualset3
107789	2	401882	13	NULL	NULL	0	NULL	Cyanothece sp	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that a diazotrophic cyanobacterium , like Cyanothece sp .
	manualset3
107790	1	401883	13	NULL	NULL	0	NULL	catabolite repression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that although catabolite repression is partly responsible for causing the inhibition of the enzyme synthesizing capacity of the cells observed immediately after gamma irradiation , the enhanced inhibition caused by incubating cells irradiated at higher doses is not due to interference with the control mechanism regulated by catabolite repression .
	manualset3
107791	2	401883	13	NULL	NULL	0	NULL	inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that although catabolite repression is partly responsible for causing the inhibition of the enzyme synthesizing capacity of the cells observed immediately after gamma irradiation , the enhanced inhibition caused by incubating cells irradiated at higher doses is not due to interference with the control mechanism regulated by catabolite repression .
	manualset3
107792	3	401883	13	NULL	NULL	0	NULL	enzyme 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that although catabolite repression is partly responsible for causing the inhibition of the enzyme synthesizing capacity of the cells observed immediately after gamma irradiation , the enhanced inhibition caused by incubating cells irradiated at higher doses is not due to interference with the control mechanism regulated by catabolite repression .
	manualset3
107793	4	401883	13	NULL	NULL	0	NULL	capacity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that although catabolite repression is partly responsible for causing the inhibition of the enzyme synthesizing capacity of the cells observed immediately after gamma irradiation , the enhanced inhibition caused by incubating cells irradiated at higher doses is not due to interference with the control mechanism regulated by catabolite repression .
	manualset3
107794	5	401883	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that although catabolite repression is partly responsible for causing the inhibition of the enzyme synthesizing capacity of the cells observed immediately after gamma irradiation , the enhanced inhibition caused by incubating cells irradiated at higher doses is not due to interference with the control mechanism regulated by catabolite repression .
	manualset3
107795	6	401883	13	NULL	NULL	0	NULL	gamma irradiation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that although catabolite repression is partly responsible for causing the inhibition of the enzyme synthesizing capacity of the cells observed immediately after gamma irradiation , the enhanced inhibition caused by incubating cells irradiated at higher doses is not due to interference with the control mechanism regulated by catabolite repression .
	manualset3
107796	7	401883	13	NULL	NULL	0	NULL	inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that although catabolite repression is partly responsible for causing the inhibition of the enzyme synthesizing capacity of the cells observed immediately after gamma irradiation , the enhanced inhibition caused by incubating cells irradiated at higher doses is not due to interference with the control mechanism regulated by catabolite repression .
	manualset3
107797	8	401883	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that although catabolite repression is partly responsible for causing the inhibition of the enzyme synthesizing capacity of the cells observed immediately after gamma irradiation , the enhanced inhibition caused by incubating cells irradiated at higher doses is not due to interference with the control mechanism regulated by catabolite repression .
	manualset3
107798	9	401883	13	NULL	NULL	0	NULL	 higher doses	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that although catabolite repression is partly responsible for causing the inhibition of the enzyme synthesizing capacity of the cells observed immediately after gamma irradiation , the enhanced inhibition caused by incubating cells irradiated at higher doses is not due to interference with the control mechanism regulated by catabolite repression .
	manualset3
107799	10	401883	13	NULL	NULL	0	NULL	interference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that although catabolite repression is partly responsible for causing the inhibition of the enzyme synthesizing capacity of the cells observed immediately after gamma irradiation , the enhanced inhibition caused by incubating cells irradiated at higher doses is not due to interference with the control mechanism regulated by catabolite repression .
	manualset3
107800	11	401883	13	NULL	NULL	NULL	NULL	control mechanism	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is suggested that although catabolite repression is partly responsible for causing the inhibition of the enzyme synthesizing capacity of the cells observed immediately after gamma irradiation , the enhanced inhibition caused by incubating cells irradiated at higher doses is not due to interference with the control mechanism regulated by catabolite repression .
	manualset3
107801	12	401883	13	NULL	NULL	0	NULL	catabolite repression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that although catabolite repression is partly responsible for causing the inhibition of the enzyme synthesizing capacity of the cells observed immediately after gamma irradiation , the enhanced inhibition caused by incubating cells irradiated at higher doses is not due to interference with the control mechanism regulated by catabolite repression .
	manualset3
107802	1	401884	13	NULL	NULL	0	NULL	artesunate	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that artesunate and artemether have moderate anthelminthic efficacy against C. sinensis in rabbits .
	manualset3
107803	2	401884	13	NULL	NULL	0	NULL	artemether 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that artesunate and artemether have moderate anthelminthic efficacy against C. sinensis in rabbits .
	manualset3
107804	3	401884	13	NULL	NULL	0	NULL	anthelminthic efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that artesunate and artemether have moderate anthelminthic efficacy against C. sinensis in rabbits .
	manualset3
107805	4	401884	13	NULL	NULL	0	NULL	C. sinensis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that artesunate and artemether have moderate anthelminthic efficacy against C. sinensis in rabbits .
	manualset3
107806	5	401884	13	NULL	NULL	0	NULL	rabbits	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that artesunate and artemether have moderate anthelminthic efficacy against C. sinensis in rabbits .
	manualset3
107807	1	401885	13	NULL	NULL	0	NULL	control 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that direct control of the effect of HBA on the immunocompetent and/or tumor cells may occur additively to or synergically with this process as the result of interaction of these compounds with the surface or intracellular receptors .
	manualset3
107808	2	401885	13	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that direct control of the effect of HBA on the immunocompetent and/or tumor cells may occur additively to or synergically with this process as the result of interaction of these compounds with the surface or intracellular receptors .
	manualset3
107809	3	401885	13	NULL	NULL	0	NULL	HBA	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that direct control of the effect of HBA on the immunocompetent and/or tumor cells may occur additively to or synergically with this process as the result of interaction of these compounds with the surface or intracellular receptors .
	manualset3
107810	4	401885	13	NULL	NULL	0	NULL	 immunocompetent cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that direct control of the effect of HBA on the immunocompetent and/or tumor cells may occur additively to or synergically with this process as the result of interaction of these compounds with the surface or intracellular receptors .
	manualset3
107811	5	401885	13	NULL	NULL	0	NULL	tumor cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that direct control of the effect of HBA on the immunocompetent and/or tumor cells may occur additively to or synergically with this process as the result of interaction of these compounds with the surface or intracellular receptors .
	manualset3
107812	6	401885	13	NULL	NULL	0	NULL	process 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that direct control of the effect of HBA on the immunocompetent and/or tumor cells may occur additively to or synergically with this process as the result of interaction of these compounds with the surface or intracellular receptors .
	manualset3
107813	7	401885	13	NULL	NULL	0	NULL	result	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that direct control of the effect of HBA on the immunocompetent and/or tumor cells may occur additively to or synergically with this process as the result of interaction of these compounds with the surface or intracellular receptors .
	manualset3
107814	8	401885	13	NULL	NULL	0	NULL	interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that direct control of the effect of HBA on the immunocompetent and/or tumor cells may occur additively to or synergically with this process as the result of interaction of these compounds with the surface or intracellular receptors .
	manualset3
107815	9	401885	13	NULL	NULL	0	NULL	compounds	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that direct control of the effect of HBA on the immunocompetent and/or tumor cells may occur additively to or synergically with this process as the result of interaction of these compounds with the surface or intracellular receptors .
	manualset3
107816	10	401885	13	NULL	NULL	0	NULL	surface receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that direct control of the effect of HBA on the immunocompetent and/or tumor cells may occur additively to or synergically with this process as the result of interaction of these compounds with the surface or intracellular receptors .
	manualset3
107817	11	401885	13	NULL	NULL	0	NULL	intracellular receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that direct control of the effect of HBA on the immunocompetent and/or tumor cells may occur additively to or synergically with this process as the result of interaction of these compounds with the surface or intracellular receptors .
	manualset3
107818	1	401886	13	NULL	NULL	0	NULL	internal release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that internal release of dopamine by the neuroendocrine system of the lungs may influence lung liquid reabsorption at birth .
	manualset3
107819	2	401886	13	NULL	NULL	0	NULL	dopamine	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that internal release of dopamine by the neuroendocrine system of the lungs may influence lung liquid reabsorption at birth .
	manualset3
107820	3	401886	13	NULL	NULL	0	NULL	neuroendocrine system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that internal release of dopamine by the neuroendocrine system of the lungs may influence lung liquid reabsorption at birth .
	manualset3
107821	4	401886	13	NULL	NULL	0	NULL	lungs 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that internal release of dopamine by the neuroendocrine system of the lungs may influence lung liquid reabsorption at birth .
	manualset3
107822	5	401886	13	NULL	NULL	0	NULL	lung liquid reabsorption	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that internal release of dopamine by the neuroendocrine system of the lungs may influence lung liquid reabsorption at birth .
	manualset3
107823	6	401886	13	NULL	NULL	0	NULL	birth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that internal release of dopamine by the neuroendocrine system of the lungs may influence lung liquid reabsorption at birth .
	manualset3
107824	1	401887	13	NULL	NULL	0	NULL	normobaric hyperoxia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that normobaric hyperoxia can induce anti-oxidant enzymes and lipid peroxidation as early as in 12th hour of hyperoxia .
	manualset3
107825	2	401887	13	NULL	NULL	0	NULL	anti-oxidant enzymes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that normobaric hyperoxia can induce anti-oxidant enzymes and lipid peroxidation as early as in 12th hour of hyperoxia .
	manualset3
107826	3	401887	13	NULL	NULL	0	NULL	lipid peroxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that normobaric hyperoxia can induce anti-oxidant enzymes and lipid peroxidation as early as in 12th hour of hyperoxia .
	manualset3
107827	4	401887	13	NULL	NULL	0	NULL	12th hour 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that normobaric hyperoxia can induce anti-oxidant enzymes and lipid peroxidation as early as in 12th hour of hyperoxia .
	manualset3
107828	5	401887	13	NULL	NULL	0	NULL	hyperoxia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that normobaric hyperoxia can induce anti-oxidant enzymes and lipid peroxidation as early as in 12th hour of hyperoxia .
	manualset3
107829	1	401888	13	NULL	NULL	0	NULL	blood pressure 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the blood pressure as well as the blood flow rate of these two vascular communications were adequate to allow performance of acute and chronic hemodialysis .
	manualset3
107830	2	401888	13	NULL	NULL	0	NULL	blood flow rate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the blood pressure as well as the blood flow rate of these two vascular communications were adequate to allow performance of acute and chronic hemodialysis .
	manualset3
107831	3	401888	13	NULL	NULL	0	NULL	two vascular communications 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the blood pressure as well as the blood flow rate of these two vascular communications were adequate to allow performance of acute and chronic hemodialysis .
	manualset3
107832	4	401888	13	NULL	NULL	0	NULL	performance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the blood pressure as well as the blood flow rate of these two vascular communications were adequate to allow performance of acute and chronic hemodialysis .
	manualset3
107833	5	401888	13	NULL	NULL	0	NULL	acute hemodialysis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the blood pressure as well as the blood flow rate of these two vascular communications were adequate to allow performance of acute and chronic hemodialysis .
	manualset3
107834	6	401888	13	NULL	NULL	0	NULL	chronic hemodialysis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the blood pressure as well as the blood flow rate of these two vascular communications were adequate to allow performance of acute and chronic hemodialysis .
	manualset3
107835	1	401889	13	NULL	NULL	0	NULL	carboxyl-terminal half 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the carboxyl-terminal half of sarcotoxin I penetrates into the bacterial membrane and that its amino-terminal half rich in basic amino acid residues interacts with acidic phospholipids in the bacterial membrane , resulting in perturbation of the membrane and loss of viability of the bacteria .
	manualset3
107836	2	401889	13	NULL	NULL	0	NULL	sarcotoxin I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the carboxyl-terminal half of sarcotoxin I penetrates into the bacterial membrane and that its amino-terminal half rich in basic amino acid residues interacts with acidic phospholipids in the bacterial membrane , resulting in perturbation of the membrane and loss of viability of the bacteria .
	manualset3
107837	3	401889	13	NULL	NULL	0	NULL	bacterial membrane	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the carboxyl-terminal half of sarcotoxin I penetrates into the bacterial membrane and that its amino-terminal half rich in basic amino acid residues interacts with acidic phospholipids in the bacterial membrane , resulting in perturbation of the membrane and loss of viability of the bacteria .
	manualset3
107838	4	401889	13	NULL	NULL	0	NULL	amino-terminal half 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the carboxyl-terminal half of sarcotoxin I penetrates into the bacterial membrane and that its amino-terminal half rich in basic amino acid residues interacts with acidic phospholipids in the bacterial membrane , resulting in perturbation of the membrane and loss of viability of the bacteria .
	manualset3
107839	5	401889	13	NULL	NULL	0	NULL	amino acid residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the carboxyl-terminal half of sarcotoxin I penetrates into the bacterial membrane and that its amino-terminal half rich in basic amino acid residues interacts with acidic phospholipids in the bacterial membrane , resulting in perturbation of the membrane and loss of viability of the bacteria .
	manualset3
107840	6	401889	13	NULL	NULL	0	NULL	phospholipids 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the carboxyl-terminal half of sarcotoxin I penetrates into the bacterial membrane and that its amino-terminal half rich in basic amino acid residues interacts with acidic phospholipids in the bacterial membrane , resulting in perturbation of the membrane and loss of viability of the bacteria .
	manualset3
107841	7	401889	13	NULL	NULL	0	NULL	bacterial membrane 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the carboxyl-terminal half of sarcotoxin I penetrates into the bacterial membrane and that its amino-terminal half rich in basic amino acid residues interacts with acidic phospholipids in the bacterial membrane , resulting in perturbation of the membrane and loss of viability of the bacteria .
	manualset3
107842	8	401889	13	NULL	NULL	0	NULL	perturbation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the carboxyl-terminal half of sarcotoxin I penetrates into the bacterial membrane and that its amino-terminal half rich in basic amino acid residues interacts with acidic phospholipids in the bacterial membrane , resulting in perturbation of the membrane and loss of viability of the bacteria .
	manualset3
107843	9	401889	13	NULL	NULL	0	NULL	membrane	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the carboxyl-terminal half of sarcotoxin I penetrates into the bacterial membrane and that its amino-terminal half rich in basic amino acid residues interacts with acidic phospholipids in the bacterial membrane , resulting in perturbation of the membrane and loss of viability of the bacteria .
	manualset3
107844	10	401889	13	NULL	NULL	0	NULL	loss of viability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the carboxyl-terminal half of sarcotoxin I penetrates into the bacterial membrane and that its amino-terminal half rich in basic amino acid residues interacts with acidic phospholipids in the bacterial membrane , resulting in perturbation of the membrane and loss of viability of the bacteria .
	manualset3
107845	11	401889	13	NULL	NULL	0	NULL	bacteria 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the carboxyl-terminal half of sarcotoxin I penetrates into the bacterial membrane and that its amino-terminal half rich in basic amino acid residues interacts with acidic phospholipids in the bacterial membrane , resulting in perturbation of the membrane and loss of viability of the bacteria .
	manualset3
107846	1	401890	13	NULL	NULL	0	NULL	cylindrical mass	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the cylindrical mass developed from six small nuclear particles .
	manualset3
107847	2	401890	13	NULL	NULL	0	NULL	six small nuclear particles	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the cylindrical mass developed from six small nuclear particles .
	manualset3
107848	1	401891	13	NULL	NULL	0	NULL	hump	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the hump of the spike potential is largely produced by a Ca-current and that the resultant increase of intracellular Ca might produce the larger AHP in C-cells , secondary to an increase in K-conductance .
	manualset3
107849	2	401891	13	NULL	NULL	0	NULL	spike potential 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the hump of the spike potential is largely produced by a Ca-current and that the resultant increase of intracellular Ca might produce the larger AHP in C-cells , secondary to an increase in K-conductance .
	manualset3
107850	3	401891	13	NULL	NULL	0	NULL	Ca-current 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the hump of the spike potential is largely produced by a Ca-current and that the resultant increase of intracellular Ca might produce the larger AHP in C-cells , secondary to an increase in K-conductance .
	manualset3
107851	4	401891	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the hump of the spike potential is largely produced by a Ca-current and that the resultant increase of intracellular Ca might produce the larger AHP in C-cells , secondary to an increase in K-conductance .
	manualset3
107852	5	401891	13	NULL	NULL	0	NULL	intracellular Ca	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the hump of the spike potential is largely produced by a Ca-current and that the resultant increase of intracellular Ca might produce the larger AHP in C-cells , secondary to an increase in K-conductance .
	manualset3
107853	6	401891	13	NULL	NULL	0	NULL	 larger AHP 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the hump of the spike potential is largely produced by a Ca-current and that the resultant increase of intracellular Ca might produce the larger AHP in C-cells , secondary to an increase in K-conductance .
	manualset3
107854	7	401891	13	NULL	NULL	0	NULL	C-cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the hump of the spike potential is largely produced by a Ca-current and that the resultant increase of intracellular Ca might produce the larger AHP in C-cells , secondary to an increase in K-conductance .
	manualset3
107855	8	401891	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the hump of the spike potential is largely produced by a Ca-current and that the resultant increase of intracellular Ca might produce the larger AHP in C-cells , secondary to an increase in K-conductance .
	manualset3
107856	9	401891	13	NULL	NULL	0	NULL	K-conductance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the hump of the spike potential is largely produced by a Ca-current and that the resultant increase of intracellular Ca might produce the larger AHP in C-cells , secondary to an increase in K-conductance .
	manualset3
107857	1	401892	13	NULL	NULL	0	NULL	susceptibilty 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the impaired susceptibilty of trophoblast to MHC nonrestricted killer cells should be functional for the survival of the semiallogeneic fetus .
	manualset3
107858	2	401892	13	NULL	NULL	0	NULL	trophoblast	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the impaired susceptibilty of trophoblast to MHC nonrestricted killer cells should be functional for the survival of the semiallogeneic fetus .
	manualset3
107859	3	401892	13	NULL	NULL	0	NULL	MHC nonrestricted killer cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the impaired susceptibilty of trophoblast to MHC nonrestricted killer cells should be functional for the survival of the semiallogeneic fetus .
	manualset3
107860	4	401892	13	NULL	NULL	0	NULL	survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the impaired susceptibilty of trophoblast to MHC nonrestricted killer cells should be functional for the survival of the semiallogeneic fetus .
	manualset3
107861	5	401892	13	NULL	NULL	0	NULL	semiallogeneic fetus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the impaired susceptibilty of trophoblast to MHC nonrestricted killer cells should be functional for the survival of the semiallogeneic fetus .
	manualset3
107862	1	401893	13	NULL	NULL	0	NULL	noradrenaline	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the infused noradrenaline retained in the spleen is largely taken up into nerve fibers and is available for subsequent release by nervous activity .
	manualset3
107863	2	401893	13	NULL	NULL	0	NULL	spleen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the infused noradrenaline retained in the spleen is largely taken up into nerve fibers and is available for subsequent release by nervous activity .
	manualset3
107864	3	401893	13	NULL	NULL	0	NULL	nerve fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the infused noradrenaline retained in the spleen is largely taken up into nerve fibers and is available for subsequent release by nervous activity .
	manualset3
107865	4	401893	13	NULL	NULL	0	NULL	subsequent release 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the infused noradrenaline retained in the spleen is largely taken up into nerve fibers and is available for subsequent release by nervous activity .
	manualset3
107866	5	401893	13	NULL	NULL	0	NULL	nervous activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the infused noradrenaline retained in the spleen is largely taken up into nerve fibers and is available for subsequent release by nervous activity .
	manualset3
107867	1	401894	13	NULL	NULL	0	NULL	matrix	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the initially produced matrix along resorbed root surfaces closely resembles that seen during initial formation of acellular extrinsic fiber cementum ( AEFC ) , whereas further apposition results in a tissue with the characteristics of CIFC .
	manualset3
107868	2	401894	13	NULL	NULL	0	NULL	root surfaces	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the initially produced matrix along resorbed root surfaces closely resembles that seen during initial formation of acellular extrinsic fiber cementum ( AEFC ) , whereas further apposition results in a tissue with the characteristics of CIFC .
	manualset3
107869	3	401894	13	NULL	NULL	0	NULL	initial formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the initially produced matrix along resorbed root surfaces closely resembles that seen during initial formation of acellular extrinsic fiber cementum ( AEFC ) , whereas further apposition results in a tissue with the characteristics of CIFC .
	manualset3
107870	4	401894	13	NULL	NULL	0	NULL	acellular extrinsic fiber cementum ( AEFC ) 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the initially produced matrix along resorbed root surfaces closely resembles that seen during initial formation of acellular extrinsic fiber cementum ( AEFC ) , whereas further apposition results in a tissue with the characteristics of CIFC .
	manualset3
107871	5	401894	13	NULL	NULL	0	NULL	apposition 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the initially produced matrix along resorbed root surfaces closely resembles that seen during initial formation of acellular extrinsic fiber cementum ( AEFC ) , whereas further apposition results in a tissue with the characteristics of CIFC .
	manualset3
107872	6	401894	13	NULL	NULL	0	NULL	results 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the initially produced matrix along resorbed root surfaces closely resembles that seen during initial formation of acellular extrinsic fiber cementum ( AEFC ) , whereas further apposition results in a tissue with the characteristics of CIFC .
	manualset3
107873	7	401894	13	NULL	NULL	0	NULL	tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the initially produced matrix along resorbed root surfaces closely resembles that seen during initial formation of acellular extrinsic fiber cementum ( AEFC ) , whereas further apposition results in a tissue with the characteristics of CIFC .
	manualset3
107874	8	401894	13	NULL	NULL	0	NULL	CIFC 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the initially produced matrix along resorbed root surfaces closely resembles that seen during initial formation of acellular extrinsic fiber cementum ( AEFC ) , whereas further apposition results in a tissue with the characteristics of CIFC .
	manualset3
107875	1	401895	13	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the relationship between plant growth strategy sensu Grime ( 1979 ) and Cs accumulation patterns may help to explain the different concentrations to which species accumulate radiocaesium from the soil .
	manualset3
107876	2	401895	13	NULL	NULL	0	NULL	plant growth strategy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the relationship between plant growth strategy sensu Grime ( 1979 ) and Cs accumulation patterns may help to explain the different concentrations to which species accumulate radiocaesium from the soil .
	manualset3
107877	3	401895	13	NULL	NULL	0	NULL	sensu Grime	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the relationship between plant growth strategy sensu Grime ( 1979 ) and Cs accumulation patterns may help to explain the different concentrations to which species accumulate radiocaesium from the soil .
	manualset3
107878	4	401895	13	NULL	NULL	0	NULL	1979	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the relationship between plant growth strategy sensu Grime ( 1979 ) and Cs accumulation patterns may help to explain the different concentrations to which species accumulate radiocaesium from the soil .
	manualset3
107879	5	401895	13	NULL	NULL	0	NULL	 Cs accumulation patterns	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the relationship between plant growth strategy sensu Grime ( 1979 ) and Cs accumulation patterns may help to explain the different concentrations to which species accumulate radiocaesium from the soil .
	manualset3
107880	6	401895	13	NULL	NULL	0	NULL	concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the relationship between plant growth strategy sensu Grime ( 1979 ) and Cs accumulation patterns may help to explain the different concentrations to which species accumulate radiocaesium from the soil .
	manualset3
107881	7	401895	13	NULL	NULL	0	NULL	species 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the relationship between plant growth strategy sensu Grime ( 1979 ) and Cs accumulation patterns may help to explain the different concentrations to which species accumulate radiocaesium from the soil .
	manualset3
107882	8	401895	13	NULL	NULL	0	NULL	radiocaesium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the relationship between plant growth strategy sensu Grime ( 1979 ) and Cs accumulation patterns may help to explain the different concentrations to which species accumulate radiocaesium from the soil .
	manualset3
107883	9	401895	13	NULL	NULL	0	NULL	soil	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the relationship between plant growth strategy sensu Grime ( 1979 ) and Cs accumulation patterns may help to explain the different concentrations to which species accumulate radiocaesium from the soil .
	manualset3
107884	1	401896	13	NULL	NULL	0	NULL	stimulating effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the stimulating effect of stress on LAF and IL-1 production possibly involves glucocorticoid hormones , as well as other stress-induced neurohumoral shifts accompanying the reaction of glucocorticoids .
	manualset3
107885	2	401896	13	NULL	NULL	0	NULL	stress	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the stimulating effect of stress on LAF and IL-1 production possibly involves glucocorticoid hormones , as well as other stress-induced neurohumoral shifts accompanying the reaction of glucocorticoids .
	manualset3
107886	3	401896	13	NULL	NULL	0	NULL	LAF production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the stimulating effect of stress on LAF and IL-1 production possibly involves glucocorticoid hormones , as well as other stress-induced neurohumoral shifts accompanying the reaction of glucocorticoids .
	manualset3
107887	4	401896	13	NULL	NULL	0	NULL	IL-1 production 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the stimulating effect of stress on LAF and IL-1 production possibly involves glucocorticoid hormones , as well as other stress-induced neurohumoral shifts accompanying the reaction of glucocorticoids .
	manualset3
107888	5	401896	13	NULL	NULL	0	NULL	glucocorticoid hormones	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the stimulating effect of stress on LAF and IL-1 production possibly involves glucocorticoid hormones , as well as other stress-induced neurohumoral shifts accompanying the reaction of glucocorticoids .
	manualset3
107889	6	401896	13	NULL	NULL	0	NULL	stress-induced neurohumoral shifts	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the stimulating effect of stress on LAF and IL-1 production possibly involves glucocorticoid hormones , as well as other stress-induced neurohumoral shifts accompanying the reaction of glucocorticoids .
	manualset3
107890	7	401896	13	NULL	NULL	0	NULL	reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the stimulating effect of stress on LAF and IL-1 production possibly involves glucocorticoid hormones , as well as other stress-induced neurohumoral shifts accompanying the reaction of glucocorticoids .
	manualset3
107891	8	401896	13	NULL	NULL	0	NULL	glucocorticoids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that the stimulating effect of stress on LAF and IL-1 production possibly involves glucocorticoid hormones , as well as other stress-induced neurohumoral shifts accompanying the reaction of glucocorticoids .
	manualset3
107892	1	401897	13	NULL	NULL	0	NULL	tubulin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that tubulin is slowly denatured in the presence of Zn2 + , exposing more binding sites .
	manualset3
107893	2	401897	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that tubulin is slowly denatured in the presence of Zn2 + , exposing more binding sites .
	manualset3
107894	3	401897	13	NULL	NULL	0	NULL	Zn2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that tubulin is slowly denatured in the presence of Zn2 + , exposing more binding sites .
	manualset3
107895	4	401897	13	NULL	NULL	0	NULL	binding sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that tubulin is slowly denatured in the presence of Zn2 + , exposing more binding sites .
	manualset3
107896	1	401898	13	NULL	NULL	0	NULL	limit stage of PFD excretion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is supposed that the limit stage of PFD excretion is a fluorocarbon transport from accumulatory organs to the lungs by lipid carriers ( lipoproteins , chylomicrons and cell membranes ) in which fluorocarbons are physically dissolved .
	manualset3
107897	2	401898	13	NULL	NULL	0	NULL	fluorocarbon transport 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is supposed that the limit stage of PFD excretion is a fluorocarbon transport from accumulatory organs to the lungs by lipid carriers ( lipoproteins , chylomicrons and cell membranes ) in which fluorocarbons are physically dissolved .
	manualset3
107898	3	401898	13	NULL	NULL	0	NULL	organs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is supposed that the limit stage of PFD excretion is a fluorocarbon transport from accumulatory organs to the lungs by lipid carriers ( lipoproteins , chylomicrons and cell membranes ) in which fluorocarbons are physically dissolved .
	manualset3
107899	4	401898	13	NULL	NULL	0	NULL	lungs 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is supposed that the limit stage of PFD excretion is a fluorocarbon transport from accumulatory organs to the lungs by lipid carriers ( lipoproteins , chylomicrons and cell membranes ) in which fluorocarbons are physically dissolved .
	manualset3
107900	5	401898	13	NULL	NULL	0	NULL	lipid carriers	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is supposed that the limit stage of PFD excretion is a fluorocarbon transport from accumulatory organs to the lungs by lipid carriers ( lipoproteins , chylomicrons and cell membranes ) in which fluorocarbons are physically dissolved .
	manualset3
107901	6	401898	13	NULL	NULL	0	NULL	lipoproteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is supposed that the limit stage of PFD excretion is a fluorocarbon transport from accumulatory organs to the lungs by lipid carriers ( lipoproteins , chylomicrons and cell membranes ) in which fluorocarbons are physically dissolved .
	manualset3
107902	7	401898	13	NULL	NULL	0	NULL	chylomicrons	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is supposed that the limit stage of PFD excretion is a fluorocarbon transport from accumulatory organs to the lungs by lipid carriers ( lipoproteins , chylomicrons and cell membranes ) in which fluorocarbons are physically dissolved .
	manualset3
107903	8	401898	13	NULL	NULL	0	NULL	cell membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	It is supposed that the limit stage of PFD excretion is a fluorocarbon transport from accumulatory organs to the lungs by lipid carriers ( lipoproteins , chylomicrons and cell membranes ) in which fluorocarbons are physically dissolved .
	manualset3
107904	9	401898	13	NULL	NULL	0	NULL	fluorocarbons	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is supposed that the limit stage of PFD excretion is a fluorocarbon transport from accumulatory organs to the lungs by lipid carriers ( lipoproteins , chylomicrons and cell membranes ) in which fluorocarbons are physically dissolved .
	manualset3
107905	1	401899	13	NULL	NULL	0	NULL	74.3 per cent 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	74.3 per cent of all reported cases were epithelial tumors ( 44.0 per cent bronchial adenomas and 30.3 per cent carcinomas ) , 15.4 per cent of embryonal and 10.3 per cent of mesenchymal origin .
	manualset3
107906	2	401899	13	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	74.3 per cent of all reported cases were epithelial tumors ( 44.0 per cent bronchial adenomas and 30.3 per cent carcinomas ) , 15.4 per cent of embryonal and 10.3 per cent of mesenchymal origin .
	manualset3
107907	3	401899	13	NULL	NULL	0	NULL	epithelial tumors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	74.3 per cent of all reported cases were epithelial tumors ( 44.0 per cent bronchial adenomas and 30.3 per cent carcinomas ) , 15.4 per cent of embryonal and 10.3 per cent of mesenchymal origin .
	manualset3
107908	4	401899	13	NULL	NULL	0	NULL	44.0 per cent	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	74.3 per cent of all reported cases were epithelial tumors ( 44.0 per cent bronchial adenomas and 30.3 per cent carcinomas ) , 15.4 per cent of embryonal and 10.3 per cent of mesenchymal origin .
	manualset3
107909	5	401899	13	NULL	NULL	0	NULL	bronchial adenomas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	74.3 per cent of all reported cases were epithelial tumors ( 44.0 per cent bronchial adenomas and 30.3 per cent carcinomas ) , 15.4 per cent of embryonal and 10.3 per cent of mesenchymal origin .
	manualset3
107910	6	401899	13	NULL	NULL	0	NULL	30.3 per cent 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	74.3 per cent of all reported cases were epithelial tumors ( 44.0 per cent bronchial adenomas and 30.3 per cent carcinomas ) , 15.4 per cent of embryonal and 10.3 per cent of mesenchymal origin .
	manualset3
107911	7	401899	13	NULL	NULL	0	NULL	carcinomas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	74.3 per cent of all reported cases were epithelial tumors ( 44.0 per cent bronchial adenomas and 30.3 per cent carcinomas ) , 15.4 per cent of embryonal and 10.3 per cent of mesenchymal origin .
	manualset3
107912	8	401899	13	NULL	NULL	0	NULL	15.4 per cent	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	74.3 per cent of all reported cases were epithelial tumors ( 44.0 per cent bronchial adenomas and 30.3 per cent carcinomas ) , 15.4 per cent of embryonal and 10.3 per cent of mesenchymal origin .
	manualset3
107913	9	401899	13	NULL	NULL	0	NULL	embryonal origin 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	74.3 per cent of all reported cases were epithelial tumors ( 44.0 per cent bronchial adenomas and 30.3 per cent carcinomas ) , 15.4 per cent of embryonal and 10.3 per cent of mesenchymal origin .
	manualset3
107914	10	401899	13	NULL	NULL	0	NULL	10.3 per cent	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	74.3 per cent of all reported cases were epithelial tumors ( 44.0 per cent bronchial adenomas and 30.3 per cent carcinomas ) , 15.4 per cent of embryonal and 10.3 per cent of mesenchymal origin .
	manualset3
107915	11	401899	13	NULL	NULL	0	NULL	mesenchymal origin	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	74.3 per cent of all reported cases were epithelial tumors ( 44.0 per cent bronchial adenomas and 30.3 per cent carcinomas ) , 15.4 per cent of embryonal and 10.3 per cent of mesenchymal origin .
	manualset3
107916	1	401900	13	NULL	NULL	0	NULL	grip position	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is the latter grip position that is actually employed and traditionally accepted in the sport of rowing .
	manualset3
107917	2	401900	13	NULL	NULL	0	NULL	sport of rowing 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is the latter grip position that is actually employed and traditionally accepted in the sport of rowing .
	manualset3
107918	1	401901	13	NULL	NULL	NULL	NULL	QBC technique	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is therefore , concluded that the QBC technique , may be appropriate for screening populations for malaria and for detection of asymptomatic carriers to control further transmission of the disease in the community .
	manualset3
107919	2	401901	13	NULL	NULL	0	NULL	screening populations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is therefore , concluded that the QBC technique , may be appropriate for screening populations for malaria and for detection of asymptomatic carriers to control further transmission of the disease in the community .
	manualset3
107920	3	401901	13	NULL	NULL	0	NULL	malaria 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It is therefore , concluded that the QBC technique , may be appropriate for screening populations for malaria and for detection of asymptomatic carriers to control further transmission of the disease in the community .
	manualset3
107921	4	401901	13	NULL	NULL	0	NULL	detection 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is therefore , concluded that the QBC technique , may be appropriate for screening populations for malaria and for detection of asymptomatic carriers to control further transmission of the disease in the community .
	manualset3
107922	5	401901	13	NULL	NULL	0	NULL	asymptomatic carriers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is therefore , concluded that the QBC technique , may be appropriate for screening populations for malaria and for detection of asymptomatic carriers to control further transmission of the disease in the community .
	manualset3
107923	6	401901	13	NULL	NULL	0	NULL	transmission	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is therefore , concluded that the QBC technique , may be appropriate for screening populations for malaria and for detection of asymptomatic carriers to control further transmission of the disease in the community .
	manualset3
107924	7	401901	13	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It is therefore , concluded that the QBC technique , may be appropriate for screening populations for malaria and for detection of asymptomatic carriers to control further transmission of the disease in the community .
	manualset3
107925	8	401901	13	NULL	NULL	0	NULL	community	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is therefore , concluded that the QBC technique , may be appropriate for screening populations for malaria and for detection of asymptomatic carriers to control further transmission of the disease in the community .
	manualset3
107926	1	401902	13	NULL	NULL	0	NULL	isoalloxazine movement	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is therefore concluded that isoalloxazine movement is required for pyridine nucleotide to gain access to the active site and for the exchange of aromatic ligands .
	manualset3
107927	2	401902	13	NULL	NULL	0	NULL	pyridine nucleotide	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It is therefore concluded that isoalloxazine movement is required for pyridine nucleotide to gain access to the active site and for the exchange of aromatic ligands .
	manualset3
107928	3	401902	13	NULL	NULL	0	NULL	 access	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is therefore concluded that isoalloxazine movement is required for pyridine nucleotide to gain access to the active site and for the exchange of aromatic ligands .
	manualset3
107929	4	401902	13	NULL	NULL	0	NULL	active site 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is therefore concluded that isoalloxazine movement is required for pyridine nucleotide to gain access to the active site and for the exchange of aromatic ligands .
	manualset3
107930	5	401902	13	NULL	NULL	0	NULL	exchange	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is therefore concluded that isoalloxazine movement is required for pyridine nucleotide to gain access to the active site and for the exchange of aromatic ligands .
	manualset3
107931	6	401902	13	NULL	NULL	0	NULL	aromatic ligands	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is therefore concluded that isoalloxazine movement is required for pyridine nucleotide to gain access to the active site and for the exchange of aromatic ligands .
	manualset3
107932	1	401903	13	NULL	NULL	0	NULL	long-term effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is therefore essential to carefully study acute and long-term effects in a preclinical state , as insulin therapy is meant to be a lifelong treatment .
	manualset3
107933	2	401903	13	NULL	NULL	0	NULL	preclinical state	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is therefore essential to carefully study acute and long-term effects in a preclinical state , as insulin therapy is meant to be a lifelong treatment .
	manualset3
107934	3	401903	13	NULL	NULL	0	NULL	insulin therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is therefore essential to carefully study acute and long-term effects in a preclinical state , as insulin therapy is meant to be a lifelong treatment .
	manualset3
107935	4	401903	13	NULL	NULL	0	NULL	lifelong treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is therefore essential to carefully study acute and long-term effects in a preclinical state , as insulin therapy is meant to be a lifelong treatment .
	manualset3
108307	5	401903	13	NULL	NULL	0	NULL	acute effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is therefore essential to carefully study acute and long-term effects in a preclinical state , as insulin therapy is meant to be a lifelong treatment .
	manualset3
107936	1	401904	13	NULL	NULL	0	NULL	rod exploration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is therefore possible that rod exploration , which is an integral part of tactile bisection , reduces neglect to such an extent that it is difficult to identify neglect in the tactile modality on this task .
	manualset3
107937	2	401904	13	NULL	NULL	0	NULL	 integral part of tactile bisection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is therefore possible that rod exploration , which is an integral part of tactile bisection , reduces neglect to such an extent that it is difficult to identify neglect in the tactile modality on this task .
	manualset3
107938	3	401904	13	NULL	NULL	0	NULL	neglect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is therefore possible that rod exploration , which is an integral part of tactile bisection , reduces neglect to such an extent that it is difficult to identify neglect in the tactile modality on this task .
	manualset3
107939	4	401904	13	NULL	NULL	0	NULL	extent 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is therefore possible that rod exploration , which is an integral part of tactile bisection , reduces neglect to such an extent that it is difficult to identify neglect in the tactile modality on this task .
	manualset3
107940	5	401904	13	NULL	NULL	0	NULL	neglect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is therefore possible that rod exploration , which is an integral part of tactile bisection , reduces neglect to such an extent that it is difficult to identify neglect in the tactile modality on this task .
	manualset3
107941	6	401904	13	NULL	NULL	0	NULL	tactile modality 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is therefore possible that rod exploration , which is an integral part of tactile bisection , reduces neglect to such an extent that it is difficult to identify neglect in the tactile modality on this task .
	manualset3
107942	7	401904	13	NULL	NULL	0	NULL	task	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is therefore possible that rod exploration , which is an integral part of tactile bisection , reduces neglect to such an extent that it is difficult to identify neglect in the tactile modality on this task .
	manualset3
107943	1	401905	13	NULL	NULL	0	NULL	transformation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is thought to promote transformation of target cells by release of growth promoting , soluble factor , perhaps a product of the viral `` tat '' gene .
	manualset3
107944	2	401905	13	NULL	NULL	0	NULL	target cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It is thought to promote transformation of target cells by release of growth promoting , soluble factor , perhaps a product of the viral `` tat '' gene .
	manualset3
107945	3	401905	13	NULL	NULL	0	NULL	release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is thought to promote transformation of target cells by release of growth promoting , soluble factor , perhaps a product of the viral `` tat '' gene .
	manualset3
107946	4	401905	13	NULL	NULL	0	NULL	growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is thought to promote transformation of target cells by release of growth promoting , soluble factor , perhaps a product of the viral `` tat '' gene .
	manualset3
107947	5	401905	13	NULL	NULL	NULL	NULL	soluble factor	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is thought to promote transformation of target cells by release of growth promoting , soluble factor , perhaps a product of the viral `` tat '' gene .
	manualset3
107948	6	401905	13	NULL	NULL	0	NULL	product	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is thought to promote transformation of target cells by release of growth promoting , soluble factor , perhaps a product of the viral `` tat '' gene .
	manualset3
107949	7	401905	13	NULL	NULL	0	NULL	viral `` tat '' gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	It is thought to promote transformation of target cells by release of growth promoting , soluble factor , perhaps a product of the viral `` tat '' gene .
	manualset3
107950	1	401906	13	NULL	NULL	0	NULL	correlations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	It is thus established that correlations between cytogenetic and molecular events can be found in CGL and ALL , as in other hemopoietic malignancies : translocation and possible rearrangement of the c-abl oncogene seem of particular importance in this case .
	manualset3
107951	2	401906	13	NULL	NULL	0	NULL	cytogenetic events	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is thus established that correlations between cytogenetic and molecular events can be found in CGL and ALL , as in other hemopoietic malignancies : translocation and possible rearrangement of the c-abl oncogene seem of particular importance in this case .
	manualset3
107952	3	401906	13	NULL	NULL	0	NULL	molecular events	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is thus established that correlations between cytogenetic and molecular events can be found in CGL and ALL , as in other hemopoietic malignancies : translocation and possible rearrangement of the c-abl oncogene seem of particular importance in this case .
	manualset3
107953	4	401906	13	NULL	NULL	0	NULL	CGL	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It is thus established that correlations between cytogenetic and molecular events can be found in CGL and ALL , as in other hemopoietic malignancies : translocation and possible rearrangement of the c-abl oncogene seem of particular importance in this case .
	manualset3
107954	5	401906	13	NULL	NULL	0	NULL	 ALL	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It is thus established that correlations between cytogenetic and molecular events can be found in CGL and ALL , as in other hemopoietic malignancies : translocation and possible rearrangement of the c-abl oncogene seem of particular importance in this case .
	manualset3
107955	6	401906	13	NULL	NULL	0	NULL	hemopoietic malignancies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is thus established that correlations between cytogenetic and molecular events can be found in CGL and ALL , as in other hemopoietic malignancies : translocation and possible rearrangement of the c-abl oncogene seem of particular importance in this case .
	manualset3
107956	7	401906	13	NULL	NULL	0	NULL	translocation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is thus established that correlations between cytogenetic and molecular events can be found in CGL and ALL , as in other hemopoietic malignancies : translocation and possible rearrangement of the c-abl oncogene seem of particular importance in this case .
	manualset3
107957	8	401906	13	NULL	NULL	0	NULL	possible rearrangement	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is thus established that correlations between cytogenetic and molecular events can be found in CGL and ALL , as in other hemopoietic malignancies : translocation and possible rearrangement of the c-abl oncogene seem of particular importance in this case .
	manualset3
107958	9	401906	13	NULL	NULL	0	NULL	c-abl oncogene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	It is thus established that correlations between cytogenetic and molecular events can be found in CGL and ALL , as in other hemopoietic malignancies : translocation and possible rearrangement of the c-abl oncogene seem of particular importance in this case .
	manualset3
107959	10	401906	13	NULL	NULL	0	NULL	importance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is thus established that correlations between cytogenetic and molecular events can be found in CGL and ALL , as in other hemopoietic malignancies : translocation and possible rearrangement of the c-abl oncogene seem of particular importance in this case .
	manualset3
107960	11	401906	13	NULL	NULL	0	NULL	case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is thus established that correlations between cytogenetic and molecular events can be found in CGL and ALL , as in other hemopoietic malignancies : translocation and possible rearrangement of the c-abl oncogene seem of particular importance in this case .
	manualset3
107961	1	401907	13	NULL	NULL	0	NULL	histidine residue	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It is thus proposed that the histidine residue is present at every benzodiazepine binding site , be it either subtype I or II .
	manualset3
107962	2	401907	13	NULL	NULL	0	NULL	benzodiazepine binding site 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is thus proposed that the histidine residue is present at every benzodiazepine binding site , be it either subtype I or II .
	manualset3
107963	3	401907	13	NULL	NULL	0	NULL	subtype I 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is thus proposed that the histidine residue is present at every benzodiazepine binding site , be it either subtype I or II .
	manualset3
107964	4	401907	13	NULL	NULL	0	NULL	subtype II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is thus proposed that the histidine residue is present at every benzodiazepine binding site , be it either subtype I or II .
	manualset3
107965	1	401908	13	NULL	NULL	0	NULL	intramuscular levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is uncertain whether intramuscular levels of coQ10 and mitochondrial function are affected by statin therapy and whether the symptoms of myopathy can be alleviated with coQ10 supplementation .
	manualset3
107966	2	401908	13	NULL	NULL	0	NULL	coQ10 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is uncertain whether intramuscular levels of coQ10 and mitochondrial function are affected by statin therapy and whether the symptoms of myopathy can be alleviated with coQ10 supplementation .
	manualset3
107967	3	401908	13	NULL	NULL	0	NULL	mitochondrial function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is uncertain whether intramuscular levels of coQ10 and mitochondrial function are affected by statin therapy and whether the symptoms of myopathy can be alleviated with coQ10 supplementation .
	manualset3
107968	4	401908	13	NULL	NULL	0	NULL	statin therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is uncertain whether intramuscular levels of coQ10 and mitochondrial function are affected by statin therapy and whether the symptoms of myopathy can be alleviated with coQ10 supplementation .
	manualset3
107969	5	401908	13	NULL	NULL	0	NULL	symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is uncertain whether intramuscular levels of coQ10 and mitochondrial function are affected by statin therapy and whether the symptoms of myopathy can be alleviated with coQ10 supplementation .
	manualset3
107970	6	401908	13	NULL	NULL	0	NULL	myopathy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is uncertain whether intramuscular levels of coQ10 and mitochondrial function are affected by statin therapy and whether the symptoms of myopathy can be alleviated with coQ10 supplementation .
	manualset3
107972	8	401908	13	NULL	NULL	NULL	NULL	coQ10 supplementation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is uncertain whether intramuscular levels of coQ10 and mitochondrial function are affected by statin therapy and whether the symptoms of myopathy can be alleviated with coQ10 supplementation .
	manualset3
107973	1	401909	13	NULL	NULL	0	NULL	metabolic responses	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is unclear whether any additional metabolic responses to leukocytic pyrogen result from prostaglandin production .
	manualset3
107974	2	401909	13	NULL	NULL	0	NULL	leukocytic pyrogen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is unclear whether any additional metabolic responses to leukocytic pyrogen result from prostaglandin production .
	manualset3
107976	4	401909	13	NULL	NULL	0	NULL	prostaglandin production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is unclear whether any additional metabolic responses to leukocytic pyrogen result from prostaglandin production .
	manualset3
107978	2	401910	13	NULL	NULL	0	NULL	clinical isolates 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	75 consecutive clinical isolates of vancomycin-resistant Enterococcus faecium ( VRE faecium ) ( 40 blood and 35 urine isolates ) isolated over 1 y at the Cleveland Clinic Foundation were tested for susceptibility to linezolid , quinupristin-dalfopristin , fosfomycin and nitrofurantoin using the Etest .
	manualset3
107979	3	401910	13	NULL	NULL	0	NULL	vancomycin-resistant Enterococcus faecium	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	75 consecutive clinical isolates of vancomycin-resistant Enterococcus faecium ( VRE faecium ) ( 40 blood and 35 urine isolates ) isolated over 1 y at the Cleveland Clinic Foundation were tested for susceptibility to linezolid , quinupristin-dalfopristin , fosfomycin and nitrofurantoin using the Etest .
	manualset3
107980	4	401910	13	NULL	NULL	0	NULL	VRE faecium 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	75 consecutive clinical isolates of vancomycin-resistant Enterococcus faecium ( VRE faecium ) ( 40 blood and 35 urine isolates ) isolated over 1 y at the Cleveland Clinic Foundation were tested for susceptibility to linezolid , quinupristin-dalfopristin , fosfomycin and nitrofurantoin using the Etest .
	manualset3
107981	5	401910	13	NULL	NULL	0	NULL	40 blood isolates 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	75 consecutive clinical isolates of vancomycin-resistant Enterococcus faecium ( VRE faecium ) ( 40 blood and 35 urine isolates ) isolated over 1 y at the Cleveland Clinic Foundation were tested for susceptibility to linezolid , quinupristin-dalfopristin , fosfomycin and nitrofurantoin using the Etest .
	manualset3
107982	6	401910	13	NULL	NULL	0	NULL	35 urine isolates	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	75 consecutive clinical isolates of vancomycin-resistant Enterococcus faecium ( VRE faecium ) ( 40 blood and 35 urine isolates ) isolated over 1 y at the Cleveland Clinic Foundation were tested for susceptibility to linezolid , quinupristin-dalfopristin , fosfomycin and nitrofurantoin using the Etest .
	manualset3
107983	7	401910	13	NULL	NULL	0	NULL	over 1 y	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	75 consecutive clinical isolates of vancomycin-resistant Enterococcus faecium ( VRE faecium ) ( 40 blood and 35 urine isolates ) isolated over 1 y at the Cleveland Clinic Foundation were tested for susceptibility to linezolid , quinupristin-dalfopristin , fosfomycin and nitrofurantoin using the Etest .
	manualset3
107984	8	401910	13	NULL	NULL	0	NULL	Cleveland Clinic Foundation	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	75 consecutive clinical isolates of vancomycin-resistant Enterococcus faecium ( VRE faecium ) ( 40 blood and 35 urine isolates ) isolated over 1 y at the Cleveland Clinic Foundation were tested for susceptibility to linezolid , quinupristin-dalfopristin , fosfomycin and nitrofurantoin using the Etest .
	manualset3
107985	9	401910	13	NULL	NULL	0	NULL	susceptibility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	75 consecutive clinical isolates of vancomycin-resistant Enterococcus faecium ( VRE faecium ) ( 40 blood and 35 urine isolates ) isolated over 1 y at the Cleveland Clinic Foundation were tested for susceptibility to linezolid , quinupristin-dalfopristin , fosfomycin and nitrofurantoin using the Etest .
	manualset3
107986	10	401910	13	NULL	NULL	0	NULL	 linezolid	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	75 consecutive clinical isolates of vancomycin-resistant Enterococcus faecium ( VRE faecium ) ( 40 blood and 35 urine isolates ) isolated over 1 y at the Cleveland Clinic Foundation were tested for susceptibility to linezolid , quinupristin-dalfopristin , fosfomycin and nitrofurantoin using the Etest .
	manualset3
107987	11	401910	13	NULL	NULL	0	NULL	quinupristin-dalfopristin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	75 consecutive clinical isolates of vancomycin-resistant Enterococcus faecium ( VRE faecium ) ( 40 blood and 35 urine isolates ) isolated over 1 y at the Cleveland Clinic Foundation were tested for susceptibility to linezolid , quinupristin-dalfopristin , fosfomycin and nitrofurantoin using the Etest .
	manualset3
107988	12	401910	13	NULL	NULL	0	NULL	fosfomycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	75 consecutive clinical isolates of vancomycin-resistant Enterococcus faecium ( VRE faecium ) ( 40 blood and 35 urine isolates ) isolated over 1 y at the Cleveland Clinic Foundation were tested for susceptibility to linezolid , quinupristin-dalfopristin , fosfomycin and nitrofurantoin using the Etest .
	manualset3
107989	13	401910	13	NULL	NULL	0	NULL	nitrofurantoin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	75 consecutive clinical isolates of vancomycin-resistant Enterococcus faecium ( VRE faecium ) ( 40 blood and 35 urine isolates ) isolated over 1 y at the Cleveland Clinic Foundation were tested for susceptibility to linezolid , quinupristin-dalfopristin , fosfomycin and nitrofurantoin using the Etest .
	manualset3
107990	14	401910	13	NULL	NULL	0	NULL	 Etest	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	75 consecutive clinical isolates of vancomycin-resistant Enterococcus faecium ( VRE faecium ) ( 40 blood and 35 urine isolates ) isolated over 1 y at the Cleveland Clinic Foundation were tested for susceptibility to linezolid , quinupristin-dalfopristin , fosfomycin and nitrofurantoin using the Etest .
	manualset3
107977	1	401911	13	NULL	NULL	NULL	NULL	cGMP signaling 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is unknown whether cGMP signaling or phosphorylation regulates the insertion of CFTR associated vesicles from the cytoplasm to the surface of enterocytes .
	manualset3
107991	2	401911	13	NULL	NULL	0	NULL	phosphorylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is unknown whether cGMP signaling or phosphorylation regulates the insertion of CFTR associated vesicles from the cytoplasm to the surface of enterocytes .
	manualset3
107992	3	401911	13	NULL	NULL	0	NULL	insertion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is unknown whether cGMP signaling or phosphorylation regulates the insertion of CFTR associated vesicles from the cytoplasm to the surface of enterocytes .
	manualset3
107993	4	401911	13	NULL	NULL	0	NULL	CFTR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It is unknown whether cGMP signaling or phosphorylation regulates the insertion of CFTR associated vesicles from the cytoplasm to the surface of enterocytes .
	manualset3
107994	5	401911	13	NULL	NULL	0	NULL	vesicles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	It is unknown whether cGMP signaling or phosphorylation regulates the insertion of CFTR associated vesicles from the cytoplasm to the surface of enterocytes .
	manualset3
107995	6	401911	13	NULL	NULL	0	NULL	cytoplasm 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	It is unknown whether cGMP signaling or phosphorylation regulates the insertion of CFTR associated vesicles from the cytoplasm to the surface of enterocytes .
	manualset3
107996	7	401911	13	NULL	NULL	0	NULL	surface of enterocytes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	It is unknown whether cGMP signaling or phosphorylation regulates the insertion of CFTR associated vesicles from the cytoplasm to the surface of enterocytes .
	manualset3
107997	1	401912	13	NULL	NULL	0	NULL	radiolucent lesion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is usually a well-defined , radiolucent lesion with a thin , sclerotic margin that varies in size from 1 cm to 4 cm ; it may contain small calcifications .
	manualset3
107998	2	401912	13	NULL	NULL	0	NULL	sclerotic margin	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is usually a well-defined , radiolucent lesion with a thin , sclerotic margin that varies in size from 1 cm to 4 cm ; it may contain small calcifications .
	manualset3
107999	3	401912	13	NULL	NULL	0	NULL	size 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is usually a well-defined , radiolucent lesion with a thin , sclerotic margin that varies in size from 1 cm to 4 cm ; it may contain small calcifications .
	manualset3
108000	4	401912	13	NULL	NULL	0	NULL	from 1 cm to 4 cm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is usually a well-defined , radiolucent lesion with a thin , sclerotic margin that varies in size from 1 cm to 4 cm ; it may contain small calcifications .
	manualset3
108001	5	401912	13	NULL	NULL	0	NULL	small calcifications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is usually a well-defined , radiolucent lesion with a thin , sclerotic margin that varies in size from 1 cm to 4 cm ; it may contain small calcifications .
	manualset3
108002	1	401913	13	NULL	NULL	0	NULL	enzyme system	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It is utilized by the enzyme system and is converted to artemisinin with the same efficiency as the natural substrates .
	manualset3
108003	2	401913	13	NULL	NULL	0	NULL	artemisinin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	It is utilized by the enzyme system and is converted to artemisinin with the same efficiency as the natural substrates .
	manualset3
108004	3	401913	13	NULL	NULL	0	NULL	efficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is utilized by the enzyme system and is converted to artemisinin with the same efficiency as the natural substrates .
	manualset3
108005	4	401913	13	NULL	NULL	0	NULL	natural substrates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is utilized by the enzyme system and is converted to artemisinin with the same efficiency as the natural substrates .
	manualset3
108006	1	401914	13	NULL	NULL	0	NULL	body fat	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is well-documented that body fat and body fat distribution are related to increased risk for cardiovascular disease , hyperinsulinemia , and diabetes mellitus .
	manualset3
108007	2	401914	13	NULL	NULL	0	NULL	body fat distribution	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is well-documented that body fat and body fat distribution are related to increased risk for cardiovascular disease , hyperinsulinemia , and diabetes mellitus .
	manualset3
108008	3	401914	13	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is well-documented that body fat and body fat distribution are related to increased risk for cardiovascular disease , hyperinsulinemia , and diabetes mellitus .
	manualset3
108009	4	401914	13	NULL	NULL	0	NULL	cardiovascular disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It is well-documented that body fat and body fat distribution are related to increased risk for cardiovascular disease , hyperinsulinemia , and diabetes mellitus .
	manualset3
108010	5	401914	13	NULL	NULL	0	NULL	hyperinsulinemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is well-documented that body fat and body fat distribution are related to increased risk for cardiovascular disease , hyperinsulinemia , and diabetes mellitus .
	manualset3
108011	6	401914	13	NULL	NULL	0	NULL	diabetes mellitus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It is well-documented that body fat and body fat distribution are related to increased risk for cardiovascular disease , hyperinsulinemia , and diabetes mellitus .
	manualset3
108012	1	401915	13	NULL	NULL	0	NULL	cancer incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is well known that cancer incidence and mortality figures are very poor in Hungary .
	manualset3
108013	2	401915	13	NULL	NULL	0	NULL	mortality figures	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It is well known that cancer incidence and mortality figures are very poor in Hungary .
	manualset3
108014	3	401915	13	NULL	NULL	0	NULL	Hungary	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	It is well known that cancer incidence and mortality figures are very poor in Hungary .
	manualset3
108015	1	401916	13	NULL	NULL	0	NULL	75Se-labeled monoclonal antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	75Se-labeled monoclonal antibodies were evaluated both in vitro and in vivo using the human osteogenic sarcoma cell line KT005 , and the results were compared with those of 125I - and 111In-labeled antibodies .
	manualset3
108016	2	401916	13	NULL	NULL	0	NULL	human osteogenic sarcoma cell line KT005	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	75Se-labeled monoclonal antibodies were evaluated both in vitro and in vivo using the human osteogenic sarcoma cell line KT005 , and the results were compared with those of 125I - and 111In-labeled antibodies .
	manualset3
108017	3	401916	13	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	75Se-labeled monoclonal antibodies were evaluated both in vitro and in vivo using the human osteogenic sarcoma cell line KT005 , and the results were compared with those of 125I - and 111In-labeled antibodies .
	manualset3
108018	4	401916	13	NULL	NULL	0	NULL	125I -labeled antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	75Se-labeled monoclonal antibodies were evaluated both in vitro and in vivo using the human osteogenic sarcoma cell line KT005 , and the results were compared with those of 125I - and 111In-labeled antibodies .
	manualset3
108019	5	401916	13	NULL	NULL	0	NULL	111In-labeled antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	75Se-labeled monoclonal antibodies were evaluated both in vitro and in vivo using the human osteogenic sarcoma cell line KT005 , and the results were compared with those of 125I - and 111In-labeled antibodies .
	manualset3
108020	1	401917	13	NULL	NULL	0	NULL	doses of 2 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It mas noted that in doses of 2 , 3 and 4 mg/kg the antibiotic had no effect on the sleep duration in mice treated with hexenal .
	manualset3
108021	2	401917	13	NULL	NULL	0	NULL	doses of 3 mg/kg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It mas noted that in doses of 2 , 3 and 4 mg/kg the antibiotic had no effect on the sleep duration in mice treated with hexenal .
	manualset3
108022	3	401917	13	NULL	NULL	0	NULL	doses of 4 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It mas noted that in doses of 2 , 3 and 4 mg/kg the antibiotic had no effect on the sleep duration in mice treated with hexenal .
	manualset3
108023	4	401917	13	NULL	NULL	0	NULL	antibiotic	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	It mas noted that in doses of 2 , 3 and 4 mg/kg the antibiotic had no effect on the sleep duration in mice treated with hexenal .
	manualset3
108024	5	401917	13	NULL	NULL	0	NULL	effect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It mas noted that in doses of 2 , 3 and 4 mg/kg the antibiotic had no effect on the sleep duration in mice treated with hexenal .
	manualset3
108025	6	401917	13	NULL	NULL	0	NULL	sleep duration 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	It mas noted that in doses of 2 , 3 and 4 mg/kg the antibiotic had no effect on the sleep duration in mice treated with hexenal .
	manualset3
108026	7	401917	13	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It mas noted that in doses of 2 , 3 and 4 mg/kg the antibiotic had no effect on the sleep duration in mice treated with hexenal .
	manualset3
108027	8	401917	13	NULL	NULL	0	NULL	hexenal	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It mas noted that in doses of 2 , 3 and 4 mg/kg the antibiotic had no effect on the sleep duration in mice treated with hexenal .
	manualset3
108028	1	401918	13	NULL	NULL	0	NULL	operator variability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It may , however , be subject to greater operator variability than sheath washing .
	manualset3
108029	2	401918	13	NULL	NULL	0	NULL	sheath washing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It may , however , be subject to greater operator variability than sheath washing .
	manualset3
108030	1	401919	13	NULL	NULL	NULL	NULL	population factors 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It may be attributable to other population factors , changes in HES coding , changes to health service organization , other biologic phenomenon , or a combination of these effects .
	manualset3
108031	2	401919	13	NULL	NULL	0	NULL	changes in HES coding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It may be attributable to other population factors , changes in HES coding , changes to health service organization , other biologic phenomenon , or a combination of these effects .
	manualset3
108032	3	401919	13	NULL	NULL	0	NULL	changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It may be attributable to other population factors , changes in HES coding , changes to health service organization , other biologic phenomenon , or a combination of these effects .
	manualset3
108033	4	401919	13	NULL	NULL	0	NULL	 health service organization	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It may be attributable to other population factors , changes in HES coding , changes to health service organization , other biologic phenomenon , or a combination of these effects .
	manualset3
108034	5	401919	13	NULL	NULL	0	NULL	biologic phenomenon	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It may be attributable to other population factors , changes in HES coding , changes to health service organization , other biologic phenomenon , or a combination of these effects .
	manualset3
108035	6	401919	13	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It may be attributable to other population factors , changes in HES coding , changes to health service organization , other biologic phenomenon , or a combination of these effects .
	manualset3
108036	7	401919	13	NULL	NULL	0	NULL	effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It may be attributable to other population factors , changes in HES coding , changes to health service organization , other biologic phenomenon , or a combination of these effects .
	manualset3
108037	1	401920	13	NULL	NULL	0	NULL	oncogene abnormalities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It may be necessary to examine oncogene abnormalities for example p53 mutation .
	manualset3
108038	2	401920	13	NULL	NULL	0	NULL	example 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It may be necessary to examine oncogene abnormalities for example p53 mutation .
	manualset3
108039	3	401920	13	NULL	NULL	0	NULL	p53 mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It may be necessary to examine oncogene abnormalities for example p53 mutation .
	manualset3
108040	1	401921	13	NULL	NULL	0	NULL	risk stratification	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It may contribute to the risk stratification and perhaps to the choice of the antithrombotic therapy in high-risk patients with elevated DD .
	manualset3
108041	2	401921	13	NULL	NULL	0	NULL	choice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It may contribute to the risk stratification and perhaps to the choice of the antithrombotic therapy in high-risk patients with elevated DD .
	manualset3
108042	3	401921	13	NULL	NULL	0	NULL	antithrombotic therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It may contribute to the risk stratification and perhaps to the choice of the antithrombotic therapy in high-risk patients with elevated DD .
	manualset3
108043	4	401921	13	NULL	NULL	0	NULL	high-risk patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It may contribute to the risk stratification and perhaps to the choice of the antithrombotic therapy in high-risk patients with elevated DD .
	manualset3
108044	5	401921	13	NULL	NULL	0	NULL	DD	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It may contribute to the risk stratification and perhaps to the choice of the antithrombotic therapy in high-risk patients with elevated DD .
	manualset3
108045	1	401922	13	NULL	NULL	0	NULL	thymic production 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It may provoke or enhance thymic production of CD4 + pathogenic self-reactive T cells by altering the thymic clonal deletion mechanism , or reduce the production of CD4 + regulatory T cells controlling self-reactive T cells , or both .
	manualset3
108046	2	401922	13	NULL	NULL	0	NULL	CD4 + pathogenic self-reactive T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It may provoke or enhance thymic production of CD4 + pathogenic self-reactive T cells by altering the thymic clonal deletion mechanism , or reduce the production of CD4 + regulatory T cells controlling self-reactive T cells , or both .
	manualset3
108047	3	401922	13	NULL	NULL	0	NULL	thymic clonal deletion mechanism 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It may provoke or enhance thymic production of CD4 + pathogenic self-reactive T cells by altering the thymic clonal deletion mechanism , or reduce the production of CD4 + regulatory T cells controlling self-reactive T cells , or both .
	manualset3
108048	4	401922	13	NULL	NULL	0	NULL	production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It may provoke or enhance thymic production of CD4 + pathogenic self-reactive T cells by altering the thymic clonal deletion mechanism , or reduce the production of CD4 + regulatory T cells controlling self-reactive T cells , or both .
	manualset3
108049	5	401922	13	NULL	NULL	0	NULL	CD4 + regulatory T cells controlling self-reactive T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It may provoke or enhance thymic production of CD4 + pathogenic self-reactive T cells by altering the thymic clonal deletion mechanism , or reduce the production of CD4 + regulatory T cells controlling self-reactive T cells , or both .
	manualset3
108050	1	401923	13	NULL	NULL	0	NULL	prophylactic activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It may therefore exert prophylactic activity in the treatment of asthma .
	manualset3
108051	2	401923	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It may therefore exert prophylactic activity in the treatment of asthma .
	manualset3
108052	3	401923	13	NULL	NULL	0	NULL	asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It may therefore exert prophylactic activity in the treatment of asthma .
	manualset3
108053	1	401924	13	NULL	NULL	0	NULL	kidney 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It may thus be concluded that the kidney , at least in part , must obtain its C ( 20 ) and C ( 22 ) fatty acids from the circulation , while the active Delta5-desaturase suggests that preformed C ( 20 ) fatty acids can be converted to more unsaturated homologs in the kidney .
	manualset3
108055	3	401924	13	NULL	NULL	0	NULL	C ( 20 ) fatty acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It may thus be concluded that the kidney , at least in part , must obtain its C ( 20 ) and C ( 22 ) fatty acids from the circulation , while the active Delta5-desaturase suggests that preformed C ( 20 ) fatty acids can be converted to more unsaturated homologs in the kidney .
	manualset3
108056	4	401924	13	NULL	NULL	0	NULL	C ( 22 ) fatty acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It may thus be concluded that the kidney , at least in part , must obtain its C ( 20 ) and C ( 22 ) fatty acids from the circulation , while the active Delta5-desaturase suggests that preformed C ( 20 ) fatty acids can be converted to more unsaturated homologs in the kidney .
	manualset3
108057	5	401924	13	NULL	NULL	0	NULL	circulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It may thus be concluded that the kidney , at least in part , must obtain its C ( 20 ) and C ( 22 ) fatty acids from the circulation , while the active Delta5-desaturase suggests that preformed C ( 20 ) fatty acids can be converted to more unsaturated homologs in the kidney .
	manualset3
108058	6	401924	13	NULL	NULL	0	NULL	 active Delta5-desaturase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It may thus be concluded that the kidney , at least in part , must obtain its C ( 20 ) and C ( 22 ) fatty acids from the circulation , while the active Delta5-desaturase suggests that preformed C ( 20 ) fatty acids can be converted to more unsaturated homologs in the kidney .
	manualset3
108059	7	401924	13	NULL	NULL	0	NULL	 C ( 20 ) fatty acids 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It may thus be concluded that the kidney , at least in part , must obtain its C ( 20 ) and C ( 22 ) fatty acids from the circulation , while the active Delta5-desaturase suggests that preformed C ( 20 ) fatty acids can be converted to more unsaturated homologs in the kidney .
	manualset3
108060	8	401924	13	NULL	NULL	0	NULL	unsaturated homologs	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It may thus be concluded that the kidney , at least in part , must obtain its C ( 20 ) and C ( 22 ) fatty acids from the circulation , while the active Delta5-desaturase suggests that preformed C ( 20 ) fatty acids can be converted to more unsaturated homologs in the kidney .
	manualset3
108061	9	401924	13	NULL	NULL	0	NULL	kidney	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It may thus be concluded that the kidney , at least in part , must obtain its C ( 20 ) and C ( 22 ) fatty acids from the circulation , while the active Delta5-desaturase suggests that preformed C ( 20 ) fatty acids can be converted to more unsaturated homologs in the kidney .
	manualset3
108062	1	401925	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It must be stressed how patients with papillary carcinoma experienced a longer postoperative survival ; it has not yet been established whether such favorable behavior is due to low biological aggressiveness or to earlier diagnosis .
	manualset3
108063	2	401925	13	NULL	NULL	0	NULL	papillary carcinoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It must be stressed how patients with papillary carcinoma experienced a longer postoperative survival ; it has not yet been established whether such favorable behavior is due to low biological aggressiveness or to earlier diagnosis .
	manualset3
108064	3	401925	13	NULL	NULL	0	NULL	postoperative survival 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It must be stressed how patients with papillary carcinoma experienced a longer postoperative survival ; it has not yet been established whether such favorable behavior is due to low biological aggressiveness or to earlier diagnosis .
	manualset3
108065	4	401925	13	NULL	NULL	0	NULL	favorable behavior	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It must be stressed how patients with papillary carcinoma experienced a longer postoperative survival ; it has not yet been established whether such favorable behavior is due to low biological aggressiveness or to earlier diagnosis .
	manualset3
108066	5	401925	13	NULL	NULL	0	NULL	low biological aggressiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It must be stressed how patients with papillary carcinoma experienced a longer postoperative survival ; it has not yet been established whether such favorable behavior is due to low biological aggressiveness or to earlier diagnosis .
	manualset3
108067	6	401925	13	NULL	NULL	0	NULL	earlier diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It must be stressed how patients with papillary carcinoma experienced a longer postoperative survival ; it has not yet been established whether such favorable behavior is due to low biological aggressiveness or to earlier diagnosis .
	manualset3
108068	1	401926	13	NULL	NULL	NULL	NULL	 professional liability  	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It must now deal with professional liability and cost containment because now there are mechanisms for the rationing of care based on costs alone .
	manualset3
108069	2	401926	13	NULL	NULL	0	NULL	cost containment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It must now deal with professional liability and cost containment because now there are mechanisms for the rationing of care based on costs alone .
	manualset3
108070	3	401926	13	NULL	NULL	NULL	NULL	mechanisms 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It must now deal with professional liability and cost containment because now there are mechanisms for the rationing of care based on costs alone .
	manualset3
108071	4	401926	13	NULL	NULL	0	NULL	rationing of care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It must now deal with professional liability and cost containment because now there are mechanisms for the rationing of care based on costs alone .
	manualset3
108072	5	401926	13	NULL	NULL	0	NULL	costs	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It must now deal with professional liability and cost containment because now there are mechanisms for the rationing of care based on costs alone .
	manualset3
108073	1	401927	13	NULL	NULL	0	NULL	role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It points out especially the role of the nurse in handling the information and the consent for the operating action , to the entrusted patient .
	manualset3
108074	2	401927	13	NULL	NULL	0	NULL	nurse 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	It points out especially the role of the nurse in handling the information and the consent for the operating action , to the entrusted patient .
	manualset3
108075	3	401927	13	NULL	NULL	0	NULL	information	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It points out especially the role of the nurse in handling the information and the consent for the operating action , to the entrusted patient .
	manualset3
108076	4	401927	13	NULL	NULL	0	NULL	consent	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It points out especially the role of the nurse in handling the information and the consent for the operating action , to the entrusted patient .
	manualset3
108077	5	401927	13	NULL	NULL	0	NULL	operating action	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It points out especially the role of the nurse in handling the information and the consent for the operating action , to the entrusted patient .
	manualset3
108078	6	401927	13	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	It points out especially the role of the nurse in handling the information and the consent for the operating action , to the entrusted patient .
	manualset3
108079	1	401928	13	NULL	NULL	0	NULL	8-epi-PGF ( 2alpha ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	8-epi-PGF ( 2alpha ) was equipotent in resistance arteries obtained from women with severely pre-eclamptic pregnancies ( EC ( 50 ) = 1.25 x10 ( -6 ) m , 0.25-6 .17 x10 ( -6 ) m ) compared with normotensive controls .
	manualset3
108080	2	401928	13	NULL	NULL	0	NULL	resistance arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	8-epi-PGF ( 2alpha ) was equipotent in resistance arteries obtained from women with severely pre-eclamptic pregnancies ( EC ( 50 ) = 1.25 x10 ( -6 ) m , 0.25-6 .17 x10 ( -6 ) m ) compared with normotensive controls .
	manualset3
108081	3	401928	13	NULL	NULL	0	NULL	women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	8-epi-PGF ( 2alpha ) was equipotent in resistance arteries obtained from women with severely pre-eclamptic pregnancies ( EC ( 50 ) = 1.25 x10 ( -6 ) m , 0.25-6 .17 x10 ( -6 ) m ) compared with normotensive controls .
	manualset3
108082	4	401928	13	NULL	NULL	0	NULL	pre-eclamptic pregnancies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	8-epi-PGF ( 2alpha ) was equipotent in resistance arteries obtained from women with severely pre-eclamptic pregnancies ( EC ( 50 ) = 1.25 x10 ( -6 ) m , 0.25-6 .17 x10 ( -6 ) m ) compared with normotensive controls .
	manualset3
108083	5	401928	13	NULL	NULL	0	NULL	EC ( 50 ) = 1.25 x10 ( -6 ) m , 0.25-6 .17 x10 ( -6 ) m 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	8-epi-PGF ( 2alpha ) was equipotent in resistance arteries obtained from women with severely pre-eclamptic pregnancies ( EC ( 50 ) = 1.25 x10 ( -6 ) m , 0.25-6 .17 x10 ( -6 ) m ) compared with normotensive controls .
	manualset3
108084	6	401928	13	NULL	NULL	0	NULL	normotensive controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	8-epi-PGF ( 2alpha ) was equipotent in resistance arteries obtained from women with severely pre-eclamptic pregnancies ( EC ( 50 ) = 1.25 x10 ( -6 ) m , 0.25-6 .17 x10 ( -6 ) m ) compared with normotensive controls .
	manualset3
108085	1	401929	13	NULL	NULL	0	NULL	DNA G + C content 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It possessed a low DNA G + C content of 31 mol % .
	manualset3
108086	2	401929	13	NULL	NULL	0	NULL	31 mol %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It possessed a low DNA G + C content of 31 mol % .
	manualset3
108087	1	401930	13	NULL	NULL	0	NULL	review	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It presents a brief review of the EA and user satisfaction and describes the development of models created during the EA .
	manualset3
108088	2	401930	13	NULL	NULL	0	NULL	 EA 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It presents a brief review of the EA and user satisfaction and describes the development of models created during the EA .
	manualset3
108089	3	401930	13	NULL	NULL	0	NULL	user satisfaction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It presents a brief review of the EA and user satisfaction and describes the development of models created during the EA .
	manualset3
108090	4	401930	13	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It presents a brief review of the EA and user satisfaction and describes the development of models created during the EA .
	manualset3
108091	5	401930	13	NULL	NULL	0	NULL	 models 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	It presents a brief review of the EA and user satisfaction and describes the development of models created during the EA .
	manualset3
108092	6	401930	13	NULL	NULL	0	NULL	 EA	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It presents a brief review of the EA and user satisfaction and describes the development of models created during the EA .
	manualset3
108966	1	401931	13	NULL	NULL	0	NULL	favorable effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It produced a favorable effect on the functional morphology of the peritoneum by leveling many morphological signs of general intoxication of the organism and in this way creating the conditions for a favorable outcome of the postoperative period .
	manualset3
108967	2	401931	13	NULL	NULL	0	NULL	functional morphology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It produced a favorable effect on the functional morphology of the peritoneum by leveling many morphological signs of general intoxication of the organism and in this way creating the conditions for a favorable outcome of the postoperative period .
	manualset3
108968	3	401931	13	NULL	NULL	0	NULL	peritoneum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It produced a favorable effect on the functional morphology of the peritoneum by leveling many morphological signs of general intoxication of the organism and in this way creating the conditions for a favorable outcome of the postoperative period .
	manualset3
108969	4	401931	13	NULL	NULL	0	NULL	leveling	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It produced a favorable effect on the functional morphology of the peritoneum by leveling many morphological signs of general intoxication of the organism and in this way creating the conditions for a favorable outcome of the postoperative period .
	manualset3
108970	5	401931	13	NULL	NULL	0	NULL	morphological signs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It produced a favorable effect on the functional morphology of the peritoneum by leveling many morphological signs of general intoxication of the organism and in this way creating the conditions for a favorable outcome of the postoperative period .
	manualset3
108971	6	401931	13	NULL	NULL	0	NULL	general intoxication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It produced a favorable effect on the functional morphology of the peritoneum by leveling many morphological signs of general intoxication of the organism and in this way creating the conditions for a favorable outcome of the postoperative period .
	manualset3
108972	7	401931	13	NULL	NULL	0	NULL	organism 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It produced a favorable effect on the functional morphology of the peritoneum by leveling many morphological signs of general intoxication of the organism and in this way creating the conditions for a favorable outcome of the postoperative period .
	manualset3
108973	8	401931	13	NULL	NULL	0	NULL	way	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It produced a favorable effect on the functional morphology of the peritoneum by leveling many morphological signs of general intoxication of the organism and in this way creating the conditions for a favorable outcome of the postoperative period .
	manualset3
108974	9	401931	13	NULL	NULL	0	NULL	conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It produced a favorable effect on the functional morphology of the peritoneum by leveling many morphological signs of general intoxication of the organism and in this way creating the conditions for a favorable outcome of the postoperative period .
	manualset3
108975	10	401931	13	NULL	NULL	0	NULL	favorable outcome 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It produced a favorable effect on the functional morphology of the peritoneum by leveling many morphological signs of general intoxication of the organism and in this way creating the conditions for a favorable outcome of the postoperative period .
	manualset3
108976	11	401931	13	NULL	NULL	0	NULL	postoperative period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	It produced a favorable effect on the functional morphology of the peritoneum by leveling many morphological signs of general intoxication of the organism and in this way creating the conditions for a favorable outcome of the postoperative period .
	manualset3
108977	1	401932	13	NULL	NULL	0	NULL	summary	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	It produces a summary scalar efficiency ratio for each DMU and identifies the amount of inefficiency .
	manualset3
108978	2	401932	13	NULL	NULL	0	NULL	scalar efficiency ratio	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It produces a summary scalar efficiency ratio for each DMU and identifies the amount of inefficiency .
	manualset3
108979	3	401932	13	NULL	NULL	0	NULL	DMU	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	It produces a summary scalar efficiency ratio for each DMU and identifies the amount of inefficiency .
	manualset3
108980	4	401932	13	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It produces a summary scalar efficiency ratio for each DMU and identifies the amount of inefficiency .
	manualset3
108981	5	401932	13	NULL	NULL	0	NULL	inefficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It produces a summary scalar efficiency ratio for each DMU and identifies the amount of inefficiency .
	manualset3
108982	1	401933	13	NULL	NULL	0	NULL	spherical pellets	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It ranges from dense spherical pellets to viscous mycelia .
	manualset3
108983	2	401933	13	NULL	NULL	0	NULL	viscous mycelia	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It ranges from dense spherical pellets to viscous mycelia .
	manualset3
108984	1	401934	13	NULL	NULL	0	NULL	54 kDa polypeptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	It reacted mainly with 54 kDa polypeptide of P.c. in EITB .
	manualset3
108985	2	401934	13	NULL	NULL	0	NULL	P.c.	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It reacted mainly with 54 kDa polypeptide of P.c. in EITB .
	manualset3
108986	3	401934	13	NULL	NULL	0	NULL	EITB	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	It reacted mainly with 54 kDa polypeptide of P.c. in EITB .
	manualset3
108987	1	401935	13	NULL	NULL	0	NULL	immobilization efficiency	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It reflects high immobilization efficiency ( approximately 23 % ) , and signal-to-noise ratio ( approximately 98 ) and resulted in high hybridization efficiency ( approximately 36 % ) in comparison to those obtained with standard methods , viz. , NTMTA ( approximately 9.76 % ) and epoxide-amine ( approximately 9.82 % ) .
	manualset3
108988	2	401935	13	NULL	NULL	0	NULL	approximately 23 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It reflects high immobilization efficiency ( approximately 23 % ) , and signal-to-noise ratio ( approximately 98 ) and resulted in high hybridization efficiency ( approximately 36 % ) in comparison to those obtained with standard methods , viz. , NTMTA ( approximately 9.76 % ) and epoxide-amine ( approximately 9.82 % ) .
	manualset3
108989	3	401935	13	NULL	NULL	0	NULL	signal-to-noise ratio 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It reflects high immobilization efficiency ( approximately 23 % ) , and signal-to-noise ratio ( approximately 98 ) and resulted in high hybridization efficiency ( approximately 36 % ) in comparison to those obtained with standard methods , viz. , NTMTA ( approximately 9.76 % ) and epoxide-amine ( approximately 9.82 % ) .
	manualset3
108990	4	401935	13	NULL	NULL	0	NULL	approximately 98	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It reflects high immobilization efficiency ( approximately 23 % ) , and signal-to-noise ratio ( approximately 98 ) and resulted in high hybridization efficiency ( approximately 36 % ) in comparison to those obtained with standard methods , viz. , NTMTA ( approximately 9.76 % ) and epoxide-amine ( approximately 9.82 % ) .
	manualset3
108991	5	401935	13	NULL	NULL	0	NULL	hybridization efficiency	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It reflects high immobilization efficiency ( approximately 23 % ) , and signal-to-noise ratio ( approximately 98 ) and resulted in high hybridization efficiency ( approximately 36 % ) in comparison to those obtained with standard methods , viz. , NTMTA ( approximately 9.76 % ) and epoxide-amine ( approximately 9.82 % ) .
	manualset3
108992	6	401935	13	NULL	NULL	0	NULL	approximately 36 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It reflects high immobilization efficiency ( approximately 23 % ) , and signal-to-noise ratio ( approximately 98 ) and resulted in high hybridization efficiency ( approximately 36 % ) in comparison to those obtained with standard methods , viz. , NTMTA ( approximately 9.76 % ) and epoxide-amine ( approximately 9.82 % ) .
	manualset3
108993	7	401935	13	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	It reflects high immobilization efficiency ( approximately 23 % ) , and signal-to-noise ratio ( approximately 98 ) and resulted in high hybridization efficiency ( approximately 36 % ) in comparison to those obtained with standard methods , viz. , NTMTA ( approximately 9.76 % ) and epoxide-amine ( approximately 9.82 % ) .
	manualset3
108994	8	401935	13	NULL	NULL	0	NULL	standard methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	It reflects high immobilization efficiency ( approximately 23 % ) , and signal-to-noise ratio ( approximately 98 ) and resulted in high hybridization efficiency ( approximately 36 % ) in comparison to those obtained with standard methods , viz. , NTMTA ( approximately 9.76 % ) and epoxide-amine ( approximately 9.82 % ) .
	manualset3
108995	9	401935	13	NULL	NULL	0	NULL	NTMTA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It reflects high immobilization efficiency ( approximately 23 % ) , and signal-to-noise ratio ( approximately 98 ) and resulted in high hybridization efficiency ( approximately 36 % ) in comparison to those obtained with standard methods , viz. , NTMTA ( approximately 9.76 % ) and epoxide-amine ( approximately 9.82 % ) .
	manualset3
108996	10	401935	13	NULL	NULL	0	NULL	approximately 9.76 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It reflects high immobilization efficiency ( approximately 23 % ) , and signal-to-noise ratio ( approximately 98 ) and resulted in high hybridization efficiency ( approximately 36 % ) in comparison to those obtained with standard methods , viz. , NTMTA ( approximately 9.76 % ) and epoxide-amine ( approximately 9.82 % ) .
	manualset3
108997	11	401935	13	NULL	NULL	0	NULL	epoxide-amine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It reflects high immobilization efficiency ( approximately 23 % ) , and signal-to-noise ratio ( approximately 98 ) and resulted in high hybridization efficiency ( approximately 36 % ) in comparison to those obtained with standard methods , viz. , NTMTA ( approximately 9.76 % ) and epoxide-amine ( approximately 9.82 % ) .
	manualset3
108998	12	401935	13	NULL	NULL	0	NULL	approximately 9.82 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It reflects high immobilization efficiency ( approximately 23 % ) , and signal-to-noise ratio ( approximately 98 ) and resulted in high hybridization efficiency ( approximately 36 % ) in comparison to those obtained with standard methods , viz. , NTMTA ( approximately 9.76 % ) and epoxide-amine ( approximately 9.82 % ) .
	manualset3
108999	1	401936	13	NULL	NULL	0	NULL	cohort of prometastatic targets	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It regulates a cohort of prometastatic targets , including FZD7 or MAP3k1 .
	manualset3
109000	2	401936	13	NULL	NULL	0	NULL	FZD7	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It regulates a cohort of prometastatic targets , including FZD7 or MAP3k1 .
	manualset3
109001	3	401936	13	NULL	NULL	0	NULL	MAP3k1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It regulates a cohort of prometastatic targets , including FZD7 or MAP3k1 .
	manualset3
109002	1	401937	13	NULL	NULL	0	NULL	ATR 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	It remains to be determined whether ATR acts directly on the channel protein or instead alters channel-bilayer interactions .
	manualset3
109003	2	401937	13	NULL	NULL	0	NULL	acts	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It remains to be determined whether ATR acts directly on the channel protein or instead alters channel-bilayer interactions .
	manualset3
109004	3	401937	13	NULL	NULL	0	NULL	channel protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It remains to be determined whether ATR acts directly on the channel protein or instead alters channel-bilayer interactions .
	manualset3
109005	4	401937	13	NULL	NULL	0	NULL	channel-bilayer interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It remains to be determined whether ATR acts directly on the channel protein or instead alters channel-bilayer interactions .
	manualset3
109006	1	401938	13	NULL	NULL	0	NULL	new class of selective factor Xa inhibitors	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	It represents a new class of selective factor Xa inhibitors without any antithrombin activity .
	manualset3
109007	2	401938	13	NULL	NULL	0	NULL	antithrombin activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It represents a new class of selective factor Xa inhibitors without any antithrombin activity .
	manualset3
109008	1	401939	13	NULL	NULL	0	NULL	pixel	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It requires a pixel located within the OD as initial information .
	manualset3
109009	2	401939	13	NULL	NULL	0	NULL	OD	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It requires a pixel located within the OD as initial information .
	manualset3
109010	3	401939	13	NULL	NULL	0	NULL	initial information	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It requires a pixel located within the OD as initial information .
	manualset3
109011	1	401940	13	NULL	NULL	0	NULL	complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It resulted in almost negligible complications in comparison to morbidity and mortality in primary caesarean section .
	manualset3
109012	2	401940	13	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	It resulted in almost negligible complications in comparison to morbidity and mortality in primary caesarean section .
	manualset3
109013	3	401940	13	NULL	NULL	0	NULL	morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It resulted in almost negligible complications in comparison to morbidity and mortality in primary caesarean section .
	manualset3
109014	4	401940	13	NULL	NULL	0	NULL	mortality 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It resulted in almost negligible complications in comparison to morbidity and mortality in primary caesarean section .
	manualset3
109015	5	401940	13	NULL	NULL	0	NULL	primary caesarean section	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It resulted in almost negligible complications in comparison to morbidity and mortality in primary caesarean section .
	manualset3
109016	1	401941	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	It reviewed data from epidemiological studies of the occupational exposure of miners and residential exposures , animal experiments and other relevant work .
	manualset3
109017	2	401941	13	NULL	NULL	0	NULL	epidemiological studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	It reviewed data from epidemiological studies of the occupational exposure of miners and residential exposures , animal experiments and other relevant work .
	manualset3
109018	3	401941	13	NULL	NULL	0	NULL	occupational exposure 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	It reviewed data from epidemiological studies of the occupational exposure of miners and residential exposures , animal experiments and other relevant work .
	manualset3
109019	4	401941	13	NULL	NULL	0	NULL	miners 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It reviewed data from epidemiological studies of the occupational exposure of miners and residential exposures , animal experiments and other relevant work .
	manualset3
109020	5	401941	13	NULL	NULL	0	NULL	residential exposures	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	It reviewed data from epidemiological studies of the occupational exposure of miners and residential exposures , animal experiments and other relevant work .
	manualset3
109021	6	401941	13	NULL	NULL	0	NULL	animal experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	It reviewed data from epidemiological studies of the occupational exposure of miners and residential exposures , animal experiments and other relevant work .
	manualset3
109022	7	401941	13	NULL	NULL	0	NULL	relevant work	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	It reviewed data from epidemiological studies of the occupational exposure of miners and residential exposures , animal experiments and other relevant work .
	manualset3
109023	1	401942	13	NULL	NULL	0	NULL	optimal ' conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	It seems , therefore , that to obtain ; optimal ' conditions for fast enzyme inactivation , the amount of heparin should be matched to plasmin rather than to antithrombin III .
	manualset3
109024	2	401942	13	NULL	NULL	0	NULL	enzyme inactivation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It seems , therefore , that to obtain ; optimal ' conditions for fast enzyme inactivation , the amount of heparin should be matched to plasmin rather than to antithrombin III .
	manualset3
109025	3	401942	13	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It seems , therefore , that to obtain ; optimal ' conditions for fast enzyme inactivation , the amount of heparin should be matched to plasmin rather than to antithrombin III .
	manualset3
109026	4	401942	13	NULL	NULL	0	NULL	heparin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	It seems , therefore , that to obtain ; optimal ' conditions for fast enzyme inactivation , the amount of heparin should be matched to plasmin rather than to antithrombin III .
	manualset3
109027	5	401942	13	NULL	NULL	0	NULL	 plasmin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It seems , therefore , that to obtain ; optimal ' conditions for fast enzyme inactivation , the amount of heparin should be matched to plasmin rather than to antithrombin III .
	manualset3
109028	6	401942	13	NULL	NULL	0	NULL	antithrombin III	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It seems , therefore , that to obtain ; optimal ' conditions for fast enzyme inactivation , the amount of heparin should be matched to plasmin rather than to antithrombin III .
	manualset3
109029	1	401943	13	NULL	NULL	0	NULL	 fatty acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It seems probable that fatty acids have to be transformed to a micellar form in order to release NTLI .
	manualset3
109030	2	401943	13	NULL	NULL	NULL	NULL	micellar form	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It seems probable that fatty acids have to be transformed to a micellar form in order to release NTLI .
	manualset3
109031	3	401943	13	NULL	NULL	0	NULL	NTLI	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It seems probable that fatty acids have to be transformed to a micellar form in order to release NTLI .
	manualset3
109032	1	401944	13	NULL	NULL	0	NULL	microRNAs 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It seems quite clear that microRNAs play important roles in neuro-oncology , as they do across perhaps all areas in biology .
	manualset3
109033	2	401944	13	NULL	NULL	0	NULL	important roles	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It seems quite clear that microRNAs play important roles in neuro-oncology , as they do across perhaps all areas in biology .
	manualset3
109034	3	401944	13	NULL	NULL	0	NULL	neuro-oncology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	It seems quite clear that microRNAs play important roles in neuro-oncology , as they do across perhaps all areas in biology .
	manualset3
109035	4	401944	13	NULL	NULL	0	NULL	all areas in biology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	It seems quite clear that microRNAs play important roles in neuro-oncology , as they do across perhaps all areas in biology .
	manualset3
109036	1	401945	13	NULL	NULL	0	NULL	undesirable affects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It seems that being aware of the undesirable affects of tamoxifen treatment during the chemotherapy and post-chemotherapy period is very important .
	manualset3
109037	2	401945	13	NULL	NULL	0	NULL	tamoxifen 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	It seems that being aware of the undesirable affects of tamoxifen treatment during the chemotherapy and post-chemotherapy period is very important .
	manualset3
109038	3	401945	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It seems that being aware of the undesirable affects of tamoxifen treatment during the chemotherapy and post-chemotherapy period is very important .
	manualset3
109039	4	401945	13	NULL	NULL	0	NULL	chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It seems that being aware of the undesirable affects of tamoxifen treatment during the chemotherapy and post-chemotherapy period is very important .
	manualset3
109040	5	401945	13	NULL	NULL	0	NULL	post-chemotherapy period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	It seems that being aware of the undesirable affects of tamoxifen treatment during the chemotherapy and post-chemotherapy period is very important .
	manualset3
109041	1	401946	13	NULL	NULL	0	NULL	exfoliative cytology	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It seems that exfoliative cytology might be a useful method for follow-up and early diagnosis of SPN in patient after laryngectomy .
	manualset3
109042	2	401946	13	NULL	NULL	0	NULL	method	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It seems that exfoliative cytology might be a useful method for follow-up and early diagnosis of SPN in patient after laryngectomy .
	manualset3
109043	3	401946	13	NULL	NULL	0	NULL	follow-up	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It seems that exfoliative cytology might be a useful method for follow-up and early diagnosis of SPN in patient after laryngectomy .
	manualset3
109044	4	401946	13	NULL	NULL	0	NULL	early diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It seems that exfoliative cytology might be a useful method for follow-up and early diagnosis of SPN in patient after laryngectomy .
	manualset3
109045	5	401946	13	NULL	NULL	0	NULL	SPN	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It seems that exfoliative cytology might be a useful method for follow-up and early diagnosis of SPN in patient after laryngectomy .
	manualset3
109046	6	401946	13	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	It seems that exfoliative cytology might be a useful method for follow-up and early diagnosis of SPN in patient after laryngectomy .
	manualset3
109047	7	401946	13	NULL	NULL	0	NULL	laryngectomy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It seems that exfoliative cytology might be a useful method for follow-up and early diagnosis of SPN in patient after laryngectomy .
	manualset3
109048	1	401947	13	NULL	NULL	0	NULL	changes of 5-HT concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It should be noted that we have never seen any changes of 5-HT concentration , tryptophan hydroxylase and monoamineoxidase activities in repeatedly ( 40 times ) immobilized rats .
	manualset3
109049	2	401947	13	NULL	NULL	0	NULL	 tryptophan hydroxylase activities 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It should be noted that we have never seen any changes of 5-HT concentration , tryptophan hydroxylase and monoamineoxidase activities in repeatedly ( 40 times ) immobilized rats .
	manualset3
109050	3	401947	13	NULL	NULL	0	NULL	monoamineoxidase activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It should be noted that we have never seen any changes of 5-HT concentration , tryptophan hydroxylase and monoamineoxidase activities in repeatedly ( 40 times ) immobilized rats .
	manualset3
109051	4	401947	13	NULL	NULL	0	NULL	40 times	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It should be noted that we have never seen any changes of 5-HT concentration , tryptophan hydroxylase and monoamineoxidase activities in repeatedly ( 40 times ) immobilized rats .
	manualset3
109052	5	401947	13	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It should be noted that we have never seen any changes of 5-HT concentration , tryptophan hydroxylase and monoamineoxidase activities in repeatedly ( 40 times ) immobilized rats .
	manualset3
109053	1	401948	13	NULL	NULL	0	NULL	86Rb +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	86Rb + uptake via the Na + , K + , Cl - cotransporter could be inhibited by other phorbol esters and by dioctanoylglycerol , an analog of diacylglycerol , but not by 4 alpha phorbol didecanoate , an ineffective activator of protein kinase C. Staurosporine , a protein kinase C inhibitor , blocked phorbol ester inhibition of 86Rb + uptake .
	manualset3
109054	2	401948	13	NULL	NULL	0	NULL	uptake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	86Rb + uptake via the Na + , K + , Cl - cotransporter could be inhibited by other phorbol esters and by dioctanoylglycerol , an analog of diacylglycerol , but not by 4 alpha phorbol didecanoate , an ineffective activator of protein kinase C. Staurosporine , a protein kinase C inhibitor , blocked phorbol ester inhibition of 86Rb + uptake .
	manualset3
109055	3	401948	13	NULL	NULL	0	NULL	 Na + , K + , Cl - cotransporter 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	86Rb + uptake via the Na + , K + , Cl - cotransporter could be inhibited by other phorbol esters and by dioctanoylglycerol , an analog of diacylglycerol , but not by 4 alpha phorbol didecanoate , an ineffective activator of protein kinase C. Staurosporine , a protein kinase C inhibitor , blocked phorbol ester inhibition of 86Rb + uptake .
	manualset3
109056	4	401948	13	NULL	NULL	0	NULL	phorbol esters	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	86Rb + uptake via the Na + , K + , Cl - cotransporter could be inhibited by other phorbol esters and by dioctanoylglycerol , an analog of diacylglycerol , but not by 4 alpha phorbol didecanoate , an ineffective activator of protein kinase C. Staurosporine , a protein kinase C inhibitor , blocked phorbol ester inhibition of 86Rb + uptake .
	manualset3
109057	5	401948	13	NULL	NULL	0	NULL	dioctanoylglycerol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	86Rb + uptake via the Na + , K + , Cl - cotransporter could be inhibited by other phorbol esters and by dioctanoylglycerol , an analog of diacylglycerol , but not by 4 alpha phorbol didecanoate , an ineffective activator of protein kinase C. Staurosporine , a protein kinase C inhibitor , blocked phorbol ester inhibition of 86Rb + uptake .
	manualset3
109058	6	401948	13	NULL	NULL	0	NULL	analog of diacylglycerol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	86Rb + uptake via the Na + , K + , Cl - cotransporter could be inhibited by other phorbol esters and by dioctanoylglycerol , an analog of diacylglycerol , but not by 4 alpha phorbol didecanoate , an ineffective activator of protein kinase C. Staurosporine , a protein kinase C inhibitor , blocked phorbol ester inhibition of 86Rb + uptake .
	manualset3
109059	7	401948	13	NULL	NULL	0	NULL	4 alpha phorbol didecanoate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	86Rb + uptake via the Na + , K + , Cl - cotransporter could be inhibited by other phorbol esters and by dioctanoylglycerol , an analog of diacylglycerol , but not by 4 alpha phorbol didecanoate , an ineffective activator of protein kinase C. Staurosporine , a protein kinase C inhibitor , blocked phorbol ester inhibition of 86Rb + uptake .
	manualset3
109060	8	401948	13	NULL	NULL	0	NULL	ineffective activator	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	86Rb + uptake via the Na + , K + , Cl - cotransporter could be inhibited by other phorbol esters and by dioctanoylglycerol , an analog of diacylglycerol , but not by 4 alpha phorbol didecanoate , an ineffective activator of protein kinase C. Staurosporine , a protein kinase C inhibitor , blocked phorbol ester inhibition of 86Rb + uptake .
	manualset3
109061	9	401948	13	NULL	NULL	0	NULL	protein kinase C	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	86Rb + uptake via the Na + , K + , Cl - cotransporter could be inhibited by other phorbol esters and by dioctanoylglycerol , an analog of diacylglycerol , but not by 4 alpha phorbol didecanoate , an ineffective activator of protein kinase C. Staurosporine , a protein kinase C inhibitor , blocked phorbol ester inhibition of 86Rb + uptake .
	manualset3
109062	10	401948	13	NULL	NULL	0	NULL	Staurosporine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	86Rb + uptake via the Na + , K + , Cl - cotransporter could be inhibited by other phorbol esters and by dioctanoylglycerol , an analog of diacylglycerol , but not by 4 alpha phorbol didecanoate , an ineffective activator of protein kinase C. Staurosporine , a protein kinase C inhibitor , blocked phorbol ester inhibition of 86Rb + uptake .
	manualset3
109063	11	401948	13	NULL	NULL	0	NULL	protein kinase C inhibitor 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	86Rb + uptake via the Na + , K + , Cl - cotransporter could be inhibited by other phorbol esters and by dioctanoylglycerol , an analog of diacylglycerol , but not by 4 alpha phorbol didecanoate , an ineffective activator of protein kinase C. Staurosporine , a protein kinase C inhibitor , blocked phorbol ester inhibition of 86Rb + uptake .
	manualset3
109064	12	401948	13	NULL	NULL	0	NULL	phorbol ester 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	86Rb + uptake via the Na + , K + , Cl - cotransporter could be inhibited by other phorbol esters and by dioctanoylglycerol , an analog of diacylglycerol , but not by 4 alpha phorbol didecanoate , an ineffective activator of protein kinase C. Staurosporine , a protein kinase C inhibitor , blocked phorbol ester inhibition of 86Rb + uptake .
	manualset3
109065	13	401948	13	NULL	NULL	0	NULL	inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	86Rb + uptake via the Na + , K + , Cl - cotransporter could be inhibited by other phorbol esters and by dioctanoylglycerol , an analog of diacylglycerol , but not by 4 alpha phorbol didecanoate , an ineffective activator of protein kinase C. Staurosporine , a protein kinase C inhibitor , blocked phorbol ester inhibition of 86Rb + uptake .
	manualset3
109066	14	401948	13	NULL	NULL	0	NULL	86Rb +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	86Rb + uptake via the Na + , K + , Cl - cotransporter could be inhibited by other phorbol esters and by dioctanoylglycerol , an analog of diacylglycerol , but not by 4 alpha phorbol didecanoate , an ineffective activator of protein kinase C. Staurosporine , a protein kinase C inhibitor , blocked phorbol ester inhibition of 86Rb + uptake .
	manualset3
109067	15	401948	13	NULL	NULL	NULL	NULL	uptake 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	86Rb + uptake via the Na + , K + , Cl - cotransporter could be inhibited by other phorbol esters and by dioctanoylglycerol , an analog of diacylglycerol , but not by 4 alpha phorbol didecanoate , an ineffective activator of protein kinase C. Staurosporine , a protein kinase C inhibitor , blocked phorbol ester inhibition of 86Rb + uptake .
	manualset3
109068	1	401949	13	NULL	NULL	0	NULL	implausible link	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	It shows that , far from being an implausible link , the relationship between dietary patterns and cancer is largely explained by the dependence of humans on their food supply -- dependence not merely in the sense of providing energy to sustain life , but more related to evolutionarily adaptive patterns of food intake and contemporary aberrations in those patterns .
	manualset3
109069	2	401949	13	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	It shows that , far from being an implausible link , the relationship between dietary patterns and cancer is largely explained by the dependence of humans on their food supply -- dependence not merely in the sense of providing energy to sustain life , but more related to evolutionarily adaptive patterns of food intake and contemporary aberrations in those patterns .
	manualset3
109070	3	401949	13	NULL	NULL	0	NULL	dietary patterns	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	It shows that , far from being an implausible link , the relationship between dietary patterns and cancer is largely explained by the dependence of humans on their food supply -- dependence not merely in the sense of providing energy to sustain life , but more related to evolutionarily adaptive patterns of food intake and contemporary aberrations in those patterns .
	manualset3
109071	4	401949	13	NULL	NULL	0	NULL	cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It shows that , far from being an implausible link , the relationship between dietary patterns and cancer is largely explained by the dependence of humans on their food supply -- dependence not merely in the sense of providing energy to sustain life , but more related to evolutionarily adaptive patterns of food intake and contemporary aberrations in those patterns .
	manualset3
109072	5	401949	13	NULL	NULL	0	NULL	dependence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It shows that , far from being an implausible link , the relationship between dietary patterns and cancer is largely explained by the dependence of humans on their food supply -- dependence not merely in the sense of providing energy to sustain life , but more related to evolutionarily adaptive patterns of food intake and contemporary aberrations in those patterns .
	manualset3
109073	6	401949	13	NULL	NULL	0	NULL	humans 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It shows that , far from being an implausible link , the relationship between dietary patterns and cancer is largely explained by the dependence of humans on their food supply -- dependence not merely in the sense of providing energy to sustain life , but more related to evolutionarily adaptive patterns of food intake and contemporary aberrations in those patterns .
	manualset3
109074	7	401949	13	NULL	NULL	NULL	NULL	food supply 	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It shows that , far from being an implausible link , the relationship between dietary patterns and cancer is largely explained by the dependence of humans on their food supply -- dependence not merely in the sense of providing energy to sustain life , but more related to evolutionarily adaptive patterns of food intake and contemporary aberrations in those patterns .
	manualset3
109076	8	401949	13	NULL	NULL	NULL	NULL	dependence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It shows that , far from being an implausible link , the relationship between dietary patterns and cancer is largely explained by the dependence of humans on their food supply -- dependence not merely in the sense of providing energy to sustain life , but more related to evolutionarily adaptive patterns of food intake and contemporary aberrations in those patterns .
	manualset3
109077	9	401949	13	NULL	NULL	0	NULL	sense	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It shows that , far from being an implausible link , the relationship between dietary patterns and cancer is largely explained by the dependence of humans on their food supply -- dependence not merely in the sense of providing energy to sustain life , but more related to evolutionarily adaptive patterns of food intake and contemporary aberrations in those patterns .
	manualset3
109078	10	401949	13	NULL	NULL	0	NULL	energy	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It shows that , far from being an implausible link , the relationship between dietary patterns and cancer is largely explained by the dependence of humans on their food supply -- dependence not merely in the sense of providing energy to sustain life , but more related to evolutionarily adaptive patterns of food intake and contemporary aberrations in those patterns .
	manualset3
109079	11	401949	13	NULL	NULL	NULL	NULL	life	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It shows that , far from being an implausible link , the relationship between dietary patterns and cancer is largely explained by the dependence of humans on their food supply -- dependence not merely in the sense of providing energy to sustain life , but more related to evolutionarily adaptive patterns of food intake and contemporary aberrations in those patterns .
	manualset3
109080	12	401949	13	NULL	NULL	0	NULL	evolutionarily adaptive patterns	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It shows that , far from being an implausible link , the relationship between dietary patterns and cancer is largely explained by the dependence of humans on their food supply -- dependence not merely in the sense of providing energy to sustain life , but more related to evolutionarily adaptive patterns of food intake and contemporary aberrations in those patterns .
	manualset3
109081	13	401949	13	NULL	NULL	0	NULL	 food intake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It shows that , far from being an implausible link , the relationship between dietary patterns and cancer is largely explained by the dependence of humans on their food supply -- dependence not merely in the sense of providing energy to sustain life , but more related to evolutionarily adaptive patterns of food intake and contemporary aberrations in those patterns .
	manualset3
109082	14	401949	13	NULL	NULL	0	NULL	contemporary aberrations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It shows that , far from being an implausible link , the relationship between dietary patterns and cancer is largely explained by the dependence of humans on their food supply -- dependence not merely in the sense of providing energy to sustain life , but more related to evolutionarily adaptive patterns of food intake and contemporary aberrations in those patterns .
	manualset3
109083	15	401949	13	NULL	NULL	0	NULL	patterns	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It shows that , far from being an implausible link , the relationship between dietary patterns and cancer is largely explained by the dependence of humans on their food supply -- dependence not merely in the sense of providing energy to sustain life , but more related to evolutionarily adaptive patterns of food intake and contemporary aberrations in those patterns .
	manualset3
109084	1	401950	13	NULL	NULL	0	NULL	derivatives of metabolites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It suggests that simple derivatives of metabolites , including neurotransmitters and cyclic nucleotides , are linked together as regulatory molecules throughout the eukaryotes .
	manualset3
109085	2	401950	13	NULL	NULL	NULL	NULL	neurotransmitters 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It suggests that simple derivatives of metabolites , including neurotransmitters and cyclic nucleotides , are linked together as regulatory molecules throughout the eukaryotes .
	manualset3
109086	3	401950	13	NULL	NULL	0	NULL	cyclic nucleotides	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It suggests that simple derivatives of metabolites , including neurotransmitters and cyclic nucleotides , are linked together as regulatory molecules throughout the eukaryotes .
	manualset3
109087	4	401950	13	NULL	NULL	0	NULL	regulatory molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	It suggests that simple derivatives of metabolites , including neurotransmitters and cyclic nucleotides , are linked together as regulatory molecules throughout the eukaryotes .
	manualset3
109088	5	401950	13	NULL	NULL	0	NULL	eukaryotes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It suggests that simple derivatives of metabolites , including neurotransmitters and cyclic nucleotides , are linked together as regulatory molecules throughout the eukaryotes .
	manualset3
109147	1	401951	13	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	It takes time and effort to apply this tool , but it is of great value for the growth and academic development of students and residents .
	manualset3
109148	2	401951	13	NULL	NULL	0	NULL	effort	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It takes time and effort to apply this tool , but it is of great value for the growth and academic development of students and residents .
	manualset3
109149	3	401951	13	NULL	NULL	0	NULL	tool	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It takes time and effort to apply this tool , but it is of great value for the growth and academic development of students and residents .
	manualset3
109150	4	401951	13	NULL	NULL	0	NULL	value 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It takes time and effort to apply this tool , but it is of great value for the growth and academic development of students and residents .
	manualset3
109151	5	401951	13	NULL	NULL	0	NULL	growth	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It takes time and effort to apply this tool , but it is of great value for the growth and academic development of students and residents .
	manualset3
109152	6	401951	13	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It takes time and effort to apply this tool , but it is of great value for the growth and academic development of students and residents .
	manualset3
109153	7	401951	13	NULL	NULL	0	NULL	students 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It takes time and effort to apply this tool , but it is of great value for the growth and academic development of students and residents .
	manualset3
109154	8	401951	13	NULL	NULL	0	NULL	residents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It takes time and effort to apply this tool , but it is of great value for the growth and academic development of students and residents .
	manualset3
109155	1	401952	13	NULL	NULL	0	NULL	Cultural Context Model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	It then describes the Cultural Context Model , developed over 15 years of experience treating domestic violence in its broader context , utilizing separate `` culture circles '' for men and women before and during couple therapy .
	manualset3
109156	2	401952	13	NULL	NULL	0	NULL	15 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	It then describes the Cultural Context Model , developed over 15 years of experience treating domestic violence in its broader context , utilizing separate `` culture circles '' for men and women before and during couple therapy .
	manualset3
109157	3	401952	13	NULL	NULL	0	NULL	experience	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It then describes the Cultural Context Model , developed over 15 years of experience treating domestic violence in its broader context , utilizing separate `` culture circles '' for men and women before and during couple therapy .
	manualset3
109158	4	401952	13	NULL	NULL	0	NULL	domestic violence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It then describes the Cultural Context Model , developed over 15 years of experience treating domestic violence in its broader context , utilizing separate `` culture circles '' for men and women before and during couple therapy .
	manualset3
109159	5	401952	13	NULL	NULL	0	NULL	context 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It then describes the Cultural Context Model , developed over 15 years of experience treating domestic violence in its broader context , utilizing separate `` culture circles '' for men and women before and during couple therapy .
	manualset3
109160	6	401952	13	NULL	NULL	0	NULL	culture circles 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It then describes the Cultural Context Model , developed over 15 years of experience treating domestic violence in its broader context , utilizing separate `` culture circles '' for men and women before and during couple therapy .
	manualset3
109161	7	401952	13	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It then describes the Cultural Context Model , developed over 15 years of experience treating domestic violence in its broader context , utilizing separate `` culture circles '' for men and women before and during couple therapy .
	manualset3
109162	8	401952	13	NULL	NULL	0	NULL	women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It then describes the Cultural Context Model , developed over 15 years of experience treating domestic violence in its broader context , utilizing separate `` culture circles '' for men and women before and during couple therapy .
	manualset3
109163	9	401952	13	NULL	NULL	0	NULL	couple therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It then describes the Cultural Context Model , developed over 15 years of experience treating domestic violence in its broader context , utilizing separate `` culture circles '' for men and women before and during couple therapy .
	manualset3
109164	1	401953	13	NULL	NULL	0	NULL	30 cm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was about 30 cm long when not preformed by an operation .
	manualset3
109165	2	401953	13	NULL	NULL	0	NULL	operation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It was about 30 cm long when not preformed by an operation .
	manualset3
109166	1	401954	13	NULL	NULL	0	NULL	Pseudomonas aeruginosa	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It was active against Pseudomonas aeruginosa ( MICs 0.5-4 mg/l ) and very active against Enterobacteriaceae .
	manualset3
109167	2	401954	13	NULL	NULL	0	NULL	MICs 0.5-4 mg/l 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was active against Pseudomonas aeruginosa ( MICs 0.5-4 mg/l ) and very active against Enterobacteriaceae .
	manualset3
109168	3	401954	13	NULL	NULL	0	NULL	Enterobacteriaceae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It was active against Pseudomonas aeruginosa ( MICs 0.5-4 mg/l ) and very active against Enterobacteriaceae .
	manualset3
109169	1	401955	13	NULL	NULL	0	NULL	preincubation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also demonstrated that preincubation of cells with resveratrol slightly diminished ATP levels despite the withdrawal of the tested compound from the buffer .
	manualset3
109170	2	401955	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also demonstrated that preincubation of cells with resveratrol slightly diminished ATP levels despite the withdrawal of the tested compound from the buffer .
	manualset3
109171	3	401955	13	NULL	NULL	0	NULL	resveratrol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also demonstrated that preincubation of cells with resveratrol slightly diminished ATP levels despite the withdrawal of the tested compound from the buffer .
	manualset3
109172	4	401955	13	NULL	NULL	0	NULL	ATP levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also demonstrated that preincubation of cells with resveratrol slightly diminished ATP levels despite the withdrawal of the tested compound from the buffer .
	manualset3
109173	5	401955	13	NULL	NULL	0	NULL	withdrawal 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also demonstrated that preincubation of cells with resveratrol slightly diminished ATP levels despite the withdrawal of the tested compound from the buffer .
	manualset3
109174	6	401955	13	NULL	NULL	0	NULL	compound 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also demonstrated that preincubation of cells with resveratrol slightly diminished ATP levels despite the withdrawal of the tested compound from the buffer .
	manualset3
109175	7	401955	13	NULL	NULL	0	NULL	buffer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also demonstrated that preincubation of cells with resveratrol slightly diminished ATP levels despite the withdrawal of the tested compound from the buffer .
	manualset3
109176	1	401956	13	NULL	NULL	0	NULL	disulfide bond	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also demonstrated that the disulfide bond found in one group of the selected peptides was crucial for 1C11 antibody recognition .
	manualset3
109177	2	401956	13	NULL	NULL	0	NULL	one group	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also demonstrated that the disulfide bond found in one group of the selected peptides was crucial for 1C11 antibody recognition .
	manualset3
109178	3	401956	13	NULL	NULL	0	NULL	peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also demonstrated that the disulfide bond found in one group of the selected peptides was crucial for 1C11 antibody recognition .
	manualset3
109179	4	401956	13	NULL	NULL	0	NULL	1C11 antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also demonstrated that the disulfide bond found in one group of the selected peptides was crucial for 1C11 antibody recognition .
	manualset3
109180	5	401956	13	NULL	NULL	0	NULL	recognition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also demonstrated that the disulfide bond found in one group of the selected peptides was crucial for 1C11 antibody recognition .
	manualset3
109181	1	401957	13	NULL	NULL	0	NULL	recombinant chlamydial sigma28	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also demonstrated that the recombinant chlamydial sigma28 does not recognize major sigma factor sigma70-consensus-like sequences in vitro .
	manualset3
109200	2	401957	13	NULL	NULL	0	NULL	sigma factor sigma70-consensus-like sequences 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also demonstrated that the recombinant chlamydial sigma28 does not recognize major sigma factor sigma70-consensus-like sequences in vitro .
	manualset3
109202	1	401958	13	NULL	NULL	0	NULL	bradykinin	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also found that bradykinin , the biologically active product of cleavage of kininogen by kallikrein , enhanced the glycosylation of IgE-binding factors .
	manualset3
109204	2	401958	13	NULL	NULL	0	NULL	active product 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also found that bradykinin , the biologically active product of cleavage of kininogen by kallikrein , enhanced the glycosylation of IgE-binding factors .
	manualset3
109207	3	401958	13	NULL	NULL	0	NULL	cleavage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also found that bradykinin , the biologically active product of cleavage of kininogen by kallikrein , enhanced the glycosylation of IgE-binding factors .
	manualset3
109208	4	401958	13	NULL	NULL	0	NULL	kininogen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also found that bradykinin , the biologically active product of cleavage of kininogen by kallikrein , enhanced the glycosylation of IgE-binding factors .
	manualset3
109209	5	401958	13	NULL	NULL	0	NULL	 kallikrein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also found that bradykinin , the biologically active product of cleavage of kininogen by kallikrein , enhanced the glycosylation of IgE-binding factors .
	manualset3
109210	6	401958	13	NULL	NULL	0	NULL	glycosylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also found that bradykinin , the biologically active product of cleavage of kininogen by kallikrein , enhanced the glycosylation of IgE-binding factors .
	manualset3
109211	7	401958	13	NULL	NULL	0	NULL	IgE-binding factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also found that bradykinin , the biologically active product of cleavage of kininogen by kallikrein , enhanced the glycosylation of IgE-binding factors .
	manualset3
109240	1	401959	13	NULL	NULL	0	NULL	PSII particles	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also found that in isolated PSII particles incubated with either pBQ or DCBQ the cyclodextrins induce only a small OE enhancement .
	manualset3
109241	2	401959	13	NULL	NULL	0	NULL	pBQ	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also found that in isolated PSII particles incubated with either pBQ or DCBQ the cyclodextrins induce only a small OE enhancement .
	manualset3
109243	3	401959	13	NULL	NULL	0	NULL	DCBQ	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also found that in isolated PSII particles incubated with either pBQ or DCBQ the cyclodextrins induce only a small OE enhancement .
	manualset3
109245	4	401959	13	NULL	NULL	0	NULL	cyclodextrins	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also found that in isolated PSII particles incubated with either pBQ or DCBQ the cyclodextrins induce only a small OE enhancement .
	manualset3
109249	5	401959	13	NULL	NULL	0	NULL	OE enhancement 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also found that in isolated PSII particles incubated with either pBQ or DCBQ the cyclodextrins induce only a small OE enhancement .
	manualset3
109260	1	401960	13	NULL	NULL	0	NULL	supervisor	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also found that supervisor social support moderated the relationship between negative emotions and work effort but not the relationship between negative emotions and CWBs .
	manualset3
109262	2	401960	13	NULL	NULL	0	NULL	social support 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also found that supervisor social support moderated the relationship between negative emotions and work effort but not the relationship between negative emotions and CWBs .
	manualset3
109264	3	401960	13	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also found that supervisor social support moderated the relationship between negative emotions and work effort but not the relationship between negative emotions and CWBs .
	manualset3
109265	4	401960	13	NULL	NULL	0	NULL	negative emotions	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also found that supervisor social support moderated the relationship between negative emotions and work effort but not the relationship between negative emotions and CWBs .
	manualset3
109266	5	401960	13	NULL	NULL	0	NULL	work effort	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also found that supervisor social support moderated the relationship between negative emotions and work effort but not the relationship between negative emotions and CWBs .
	manualset3
109268	6	401960	13	NULL	NULL	0	NULL	relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also found that supervisor social support moderated the relationship between negative emotions and work effort but not the relationship between negative emotions and CWBs .
	manualset3
109270	7	401960	13	NULL	NULL	0	NULL	negative emotions	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also found that supervisor social support moderated the relationship between negative emotions and work effort but not the relationship between negative emotions and CWBs .
	manualset3
109272	8	401960	13	NULL	NULL	0	NULL	CWBs 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also found that supervisor social support moderated the relationship between negative emotions and work effort but not the relationship between negative emotions and CWBs .
	manualset3
109277	1	401961	13	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It was apparent that the animals used the EPS as a source of energy and nutrition .
	manualset3
109284	2	401961	13	NULL	NULL	0	NULL	EPS	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was apparent that the animals used the EPS as a source of energy and nutrition .
	manualset3
109285	3	401961	13	NULL	NULL	NULL	NULL	source of energy	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was apparent that the animals used the EPS as a source of energy and nutrition .
	manualset3
109287	5	401961	13	NULL	NULL	0	NULL	nutrition	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	It was apparent that the animals used the EPS as a source of energy and nutrition .
	manualset3
109301	1	401962	13	NULL	NULL	0	NULL	CT	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was assumed that free CT arose in the lower gastrointestinal tract from protein-CT and fibre-CT dissociation to be digested and/or absorbed .
	manualset3
109302	2	401962	13	NULL	NULL	0	NULL	lower gastrointestinal tract 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It was assumed that free CT arose in the lower gastrointestinal tract from protein-CT and fibre-CT dissociation to be digested and/or absorbed .
	manualset3
109303	3	401962	13	NULL	NULL	NULL	NULL	protein-CT dissociation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was assumed that free CT arose in the lower gastrointestinal tract from protein-CT and fibre-CT dissociation to be digested and/or absorbed .
	manualset3
109304	4	401962	13	NULL	NULL	0	NULL	fibre-CT dissociation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was assumed that free CT arose in the lower gastrointestinal tract from protein-CT and fibre-CT dissociation to be digested and/or absorbed .
	manualset3
109305	1	401963	13	NULL	NULL	0	NULL	89 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	89 preschool children , 2-4 years old , treated under the diagnosis of appendicitis were analyzed , 46 of them were operated .
	manualset3
109306	2	401963	13	NULL	NULL	0	NULL	preschool children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	89 preschool children , 2-4 years old , treated under the diagnosis of appendicitis were analyzed , 46 of them were operated .
	manualset3
109307	3	401963	13	NULL	NULL	0	NULL	2-4 years old	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	89 preschool children , 2-4 years old , treated under the diagnosis of appendicitis were analyzed , 46 of them were operated .
	manualset3
109308	4	401963	13	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	89 preschool children , 2-4 years old , treated under the diagnosis of appendicitis were analyzed , 46 of them were operated .
	manualset3
109349	5	401963	13	NULL	NULL	0	NULL	appendicitis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	89 preschool children , 2-4 years old , treated under the diagnosis of appendicitis were analyzed , 46 of them were operated .
	manualset3
109350	6	401963	13	NULL	NULL	0	NULL	46 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	89 preschool children , 2-4 years old , treated under the diagnosis of appendicitis were analyzed , 46 of them were operated .
	manualset3
109351	1	401964	13	NULL	NULL	0	NULL	surface oxide	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	It was clear that the surface oxide governs the electrode reactions .
	manualset3
109352	2	401964	13	NULL	NULL	0	NULL	electrode	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It was clear that the surface oxide governs the electrode reactions .
	manualset3
109353	3	401964	13	NULL	NULL	0	NULL	reactions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was clear that the surface oxide governs the electrode reactions .
	manualset3
109354	1	401965	13	NULL	NULL	0	NULL	man	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that , in man , infusion of a non hypotensive dose of hANP is followed by a rise in urinary PG excretion presumably reflecting enhanced renal PG biosynthesis .
	manualset3
109355	2	401965	13	NULL	NULL	0	NULL	infusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that , in man , infusion of a non hypotensive dose of hANP is followed by a rise in urinary PG excretion presumably reflecting enhanced renal PG biosynthesis .
	manualset3
109356	3	401965	13	NULL	NULL	0	NULL	hypotensive dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that , in man , infusion of a non hypotensive dose of hANP is followed by a rise in urinary PG excretion presumably reflecting enhanced renal PG biosynthesis .
	manualset3
109357	4	401965	13	NULL	NULL	0	NULL	hANP	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that , in man , infusion of a non hypotensive dose of hANP is followed by a rise in urinary PG excretion presumably reflecting enhanced renal PG biosynthesis .
	manualset3
109358	5	401965	13	NULL	NULL	0	NULL	 rise in urinary PG excretion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that , in man , infusion of a non hypotensive dose of hANP is followed by a rise in urinary PG excretion presumably reflecting enhanced renal PG biosynthesis .
	manualset3
109359	6	401965	13	NULL	NULL	0	NULL	renal PG biosynthesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that , in man , infusion of a non hypotensive dose of hANP is followed by a rise in urinary PG excretion presumably reflecting enhanced renal PG biosynthesis .
	manualset3
109360	1	401966	13	NULL	NULL	0	NULL	Group-B	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that : Group-B has been superior to Group-A .
	manualset3
109361	2	401966	13	NULL	NULL	0	NULL	Group-A	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that : Group-B has been superior to Group-A .
	manualset3
109362	1	401967	13	NULL	NULL	0	NULL	activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that activation of radiation-induced G2 arrest sensitizes osteoblasts to agents that mediate apoptosis through a mitochondrial-dependent death pathway .
	manualset3
109363	2	401967	13	NULL	NULL	0	NULL	G2 arrest	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that activation of radiation-induced G2 arrest sensitizes osteoblasts to agents that mediate apoptosis through a mitochondrial-dependent death pathway .
	manualset3
109364	3	401967	13	NULL	NULL	0	NULL	osteoblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that activation of radiation-induced G2 arrest sensitizes osteoblasts to agents that mediate apoptosis through a mitochondrial-dependent death pathway .
	manualset3
109365	4	401967	13	NULL	NULL	0	NULL	agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that activation of radiation-induced G2 arrest sensitizes osteoblasts to agents that mediate apoptosis through a mitochondrial-dependent death pathway .
	manualset3
109366	5	401967	13	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that activation of radiation-induced G2 arrest sensitizes osteoblasts to agents that mediate apoptosis through a mitochondrial-dependent death pathway .
	manualset3
109367	6	401967	13	NULL	NULL	0	NULL	mitochondrial-dependent death pathway 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that activation of radiation-induced G2 arrest sensitizes osteoblasts to agents that mediate apoptosis through a mitochondrial-dependent death pathway .
	manualset3
109368	1	401968	13	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that exposure to acute bed-rest conditions induces significantly greater urinary and serum calcium changes than rigorous bed-rest conditions in endurance trained volunteers .
	manualset3
109369	2	401968	13	NULL	NULL	0	NULL	acute bed-rest conditions 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that exposure to acute bed-rest conditions induces significantly greater urinary and serum calcium changes than rigorous bed-rest conditions in endurance trained volunteers .
	manualset3
109370	3	401968	13	NULL	NULL	0	NULL	urinary changes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that exposure to acute bed-rest conditions induces significantly greater urinary and serum calcium changes than rigorous bed-rest conditions in endurance trained volunteers .
	manualset3
109371	4	401968	13	NULL	NULL	0	NULL	serum calcium changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that exposure to acute bed-rest conditions induces significantly greater urinary and serum calcium changes than rigorous bed-rest conditions in endurance trained volunteers .
	manualset3
109372	5	401968	13	NULL	NULL	0	NULL	rigorous bed-rest conditions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that exposure to acute bed-rest conditions induces significantly greater urinary and serum calcium changes than rigorous bed-rest conditions in endurance trained volunteers .
	manualset3
109373	6	401968	13	NULL	NULL	0	NULL	endurance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that exposure to acute bed-rest conditions induces significantly greater urinary and serum calcium changes than rigorous bed-rest conditions in endurance trained volunteers .
	manualset3
109374	7	401968	13	NULL	NULL	0	NULL	trained volunteers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that exposure to acute bed-rest conditions induces significantly greater urinary and serum calcium changes than rigorous bed-rest conditions in endurance trained volunteers .
	manualset3
109375	1	401969	13	NULL	NULL	0	NULL	social contact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that reduced social contact ( i.e. , individual housing ) with subsequent exposure to an acute stressor does not appear to inhibit immunological responsiveness to an antigen .
	manualset3
109376	2	401969	13	NULL	NULL	0	NULL	individual housing 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that reduced social contact ( i.e. , individual housing ) with subsequent exposure to an acute stressor does not appear to inhibit immunological responsiveness to an antigen .
	manualset3
109377	3	401969	13	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that reduced social contact ( i.e. , individual housing ) with subsequent exposure to an acute stressor does not appear to inhibit immunological responsiveness to an antigen .
	manualset3
109378	4	401969	13	NULL	NULL	0	NULL	acute stressor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that reduced social contact ( i.e. , individual housing ) with subsequent exposure to an acute stressor does not appear to inhibit immunological responsiveness to an antigen .
	manualset3
109379	5	401969	13	NULL	NULL	0	NULL	immunological responsiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that reduced social contact ( i.e. , individual housing ) with subsequent exposure to an acute stressor does not appear to inhibit immunological responsiveness to an antigen .
	manualset3
109380	6	401969	13	NULL	NULL	0	NULL	antigen	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that reduced social contact ( i.e. , individual housing ) with subsequent exposure to an acute stressor does not appear to inhibit immunological responsiveness to an antigen .
	manualset3
109381	1	401970	13	NULL	NULL	0	NULL	students 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that students can make a very meaningful contribution to program design .
	manualset3
109382	2	401970	13	NULL	NULL	0	NULL	contribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that students can make a very meaningful contribution to program design .
	manualset3
109383	3	401970	13	NULL	NULL	0	NULL	program design 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that students can make a very meaningful contribution to program design .
	manualset3
109384	1	401971	13	NULL	NULL	0	NULL	Syrian hamster	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the Syrian hamster is more susceptible to the papillotoxic effects of diphenylamine than the Sprague-Dawley rat and the Mongolian gerbil .
	manualset3
109385	2	401971	13	NULL	NULL	0	NULL	papillotoxic effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the Syrian hamster is more susceptible to the papillotoxic effects of diphenylamine than the Sprague-Dawley rat and the Mongolian gerbil .
	manualset3
109386	3	401971	13	NULL	NULL	0	NULL	diphenylamine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the Syrian hamster is more susceptible to the papillotoxic effects of diphenylamine than the Sprague-Dawley rat and the Mongolian gerbil .
	manualset3
109387	4	401971	13	NULL	NULL	0	NULL	Sprague-Dawley rat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the Syrian hamster is more susceptible to the papillotoxic effects of diphenylamine than the Sprague-Dawley rat and the Mongolian gerbil .
	manualset3
109388	5	401971	13	NULL	NULL	0	NULL	Mongolian gerbil	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the Syrian hamster is more susceptible to the papillotoxic effects of diphenylamine than the Sprague-Dawley rat and the Mongolian gerbil .
	manualset3
109389	1	401972	13	NULL	NULL	0	NULL	interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the above interactions entail structural changes in the complexes formed , which trigger the activator , increase the rate constants of low molecular weight substrates but create steric hindrances to the interaction with protein substrates and inhibitors .
	manualset3
109390	2	401972	13	NULL	NULL	0	NULL	structural changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the above interactions entail structural changes in the complexes formed , which trigger the activator , increase the rate constants of low molecular weight substrates but create steric hindrances to the interaction with protein substrates and inhibitors .
	manualset3
109391	3	401972	13	NULL	NULL	0	NULL	complexes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the above interactions entail structural changes in the complexes formed , which trigger the activator , increase the rate constants of low molecular weight substrates but create steric hindrances to the interaction with protein substrates and inhibitors .
	manualset3
109393	5	401972	13	NULL	NULL	NULL	NULL	activator	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was concluded that the above interactions entail structural changes in the complexes formed , which trigger the activator , increase the rate constants of low molecular weight substrates but create steric hindrances to the interaction with protein substrates and inhibitors .
	manualset3
109395	7	401972	13	NULL	NULL	0	NULL	rate constants	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the above interactions entail structural changes in the complexes formed , which trigger the activator , increase the rate constants of low molecular weight substrates but create steric hindrances to the interaction with protein substrates and inhibitors .
	manualset3
109396	8	401972	13	NULL	NULL	0	NULL	low molecular weight substrates	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the above interactions entail structural changes in the complexes formed , which trigger the activator , increase the rate constants of low molecular weight substrates but create steric hindrances to the interaction with protein substrates and inhibitors .
	manualset3
109397	9	401972	13	NULL	NULL	0	NULL	steric hindrances 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the above interactions entail structural changes in the complexes formed , which trigger the activator , increase the rate constants of low molecular weight substrates but create steric hindrances to the interaction with protein substrates and inhibitors .
	manualset3
109398	10	401972	13	NULL	NULL	0	NULL	interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the above interactions entail structural changes in the complexes formed , which trigger the activator , increase the rate constants of low molecular weight substrates but create steric hindrances to the interaction with protein substrates and inhibitors .
	manualset3
109399	11	401972	13	NULL	NULL	0	NULL	protein substrates	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the above interactions entail structural changes in the complexes formed , which trigger the activator , increase the rate constants of low molecular weight substrates but create steric hindrances to the interaction with protein substrates and inhibitors .
	manualset3
109400	12	401972	13	NULL	NULL	0	NULL	protein inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the above interactions entail structural changes in the complexes formed , which trigger the activator , increase the rate constants of low molecular weight substrates but create steric hindrances to the interaction with protein substrates and inhibitors .
	manualset3
109401	1	401973	13	NULL	NULL	0	NULL	89K precursor proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	89K precursor proteins of 32K , 41.5 K , and 52K were detected .
	manualset3
109402	2	401973	13	NULL	NULL	0	NULL	32K	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	89K precursor proteins of 32K , 41.5 K , and 52K were detected .
	manualset3
109403	3	401973	13	NULL	NULL	0	NULL	41.5 K	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	89K precursor proteins of 32K , 41.5 K , and 52K were detected .
	manualset3
109404	4	401973	13	NULL	NULL	0	NULL	52K 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	89K precursor proteins of 32K , 41.5 K , and 52K were detected .
	manualset3
109405	1	401974	13	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the effect of delay frequency on the forgetting function is mediated by the effect of the reinforcer distribution , which influences discriminability by weakening stimulus control .
	manualset3
109406	2	401974	13	NULL	NULL	0	NULL	delay 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the effect of delay frequency on the forgetting function is mediated by the effect of the reinforcer distribution , which influences discriminability by weakening stimulus control .
	manualset3
109407	3	401974	13	NULL	NULL	0	NULL	frequency	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the effect of delay frequency on the forgetting function is mediated by the effect of the reinforcer distribution , which influences discriminability by weakening stimulus control .
	manualset3
109408	4	401974	13	NULL	NULL	0	NULL	function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the effect of delay frequency on the forgetting function is mediated by the effect of the reinforcer distribution , which influences discriminability by weakening stimulus control .
	manualset3
109409	5	401974	13	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the effect of delay frequency on the forgetting function is mediated by the effect of the reinforcer distribution , which influences discriminability by weakening stimulus control .
	manualset3
109410	6	401974	13	NULL	NULL	0	NULL	reinforcer distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the effect of delay frequency on the forgetting function is mediated by the effect of the reinforcer distribution , which influences discriminability by weakening stimulus control .
	manualset3
109412	7	401974	13	NULL	NULL	0	NULL	weakening stimulus control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the effect of delay frequency on the forgetting function is mediated by the effect of the reinforcer distribution , which influences discriminability by weakening stimulus control .
	manualset3
112983	8	401974	13	NULL	NULL	0	NULL	discriminability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the effect of delay frequency on the forgetting function is mediated by the effect of the reinforcer distribution , which influences discriminability by weakening stimulus control .
	manualset3
109413	1	401975	13	NULL	NULL	0	NULL	endotoxin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the endotoxin could enhance percentage of survival against E. tarda infection in Singhi .
	manualset3
109414	2	401975	13	NULL	NULL	0	NULL	percentage	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the endotoxin could enhance percentage of survival against E. tarda infection in Singhi .
	manualset3
109415	3	401975	13	NULL	NULL	0	NULL	survival 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the endotoxin could enhance percentage of survival against E. tarda infection in Singhi .
	manualset3
109416	4	401975	13	NULL	NULL	0	NULL	E. tarda	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the endotoxin could enhance percentage of survival against E. tarda infection in Singhi .
	manualset3
109417	5	401975	13	NULL	NULL	0	NULL	infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the endotoxin could enhance percentage of survival against E. tarda infection in Singhi .
	manualset3
109418	6	401975	13	NULL	NULL	0	NULL	Singhi 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the endotoxin could enhance percentage of survival against E. tarda infection in Singhi .
	manualset3
109419	1	401976	13	NULL	NULL	NULL	NULL	muscle function	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was concluded that the greater muscle function and morphology , the lower electrolyte and water deposition , the higher water and electrolyte losses , and the lower water and electrolyte content .
	manualset3
109420	2	401976	13	NULL	NULL	0	NULL	muscle morphology	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the greater muscle function and morphology , the lower electrolyte and water deposition , the higher water and electrolyte losses , and the lower water and electrolyte content .
	manualset3
109421	3	401976	13	NULL	NULL	NULL	NULL	electrolyte deposition	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was concluded that the greater muscle function and morphology , the lower electrolyte and water deposition , the higher water and electrolyte losses , and the lower water and electrolyte content .
	manualset3
109422	4	401976	13	NULL	NULL	NULL	NULL	water deposition	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was concluded that the greater muscle function and morphology , the lower electrolyte and water deposition , the higher water and electrolyte losses , and the lower water and electrolyte content .
	manualset3
109423	5	401976	13	NULL	NULL	NULL	NULL	water losses	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was concluded that the greater muscle function and morphology , the lower electrolyte and water deposition , the higher water and electrolyte losses , and the lower water and electrolyte content .
	manualset3
109424	6	401976	13	NULL	NULL	NULL	NULL	electrolyte losses	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was concluded that the greater muscle function and morphology , the lower electrolyte and water deposition , the higher water and electrolyte losses , and the lower water and electrolyte content .
	manualset3
109425	7	401976	13	NULL	NULL	0	NULL	water content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the greater muscle function and morphology , the lower electrolyte and water deposition , the higher water and electrolyte losses , and the lower water and electrolyte content .
	manualset3
109426	8	401976	13	NULL	NULL	0	NULL	electrolyte content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that the greater muscle function and morphology , the lower electrolyte and water deposition , the higher water and electrolyte losses , and the lower water and electrolyte content .
	manualset3
109427	1	401977	13	NULL	NULL	0	NULL	zinc	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that zinc played an important role on maintaining the normal activities of Na + , K ( + ) - ATPase and Ca2 + , Mg ( 2 + ) - ATPase .
	manualset3
109428	2	401977	13	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that zinc played an important role on maintaining the normal activities of Na + , K ( + ) - ATPase and Ca2 + , Mg ( 2 + ) - ATPase .
	manualset3
109429	3	401977	13	NULL	NULL	0	NULL	activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that zinc played an important role on maintaining the normal activities of Na + , K ( + ) - ATPase and Ca2 + , Mg ( 2 + ) - ATPase .
	manualset3
109430	4	401977	13	NULL	NULL	NULL	NULL	Na + , K ( + ) - ATPase 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was concluded that zinc played an important role on maintaining the normal activities of Na + , K ( + ) - ATPase and Ca2 + , Mg ( 2 + ) - ATPase .
	manualset3
109431	5	401977	13	NULL	NULL	NULL	NULL	Ca2 + , Mg ( 2 + ) - ATPase	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was concluded that zinc played an important role on maintaining the normal activities of Na + , K ( + ) - ATPase and Ca2 + , Mg ( 2 + ) - ATPase .
	manualset3
109434	1	401978	13	NULL	NULL	0	NULL	 rational truncation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was constructed by rational truncation of GBD-CD2 , which harbors the second catalytic domain of DSR-E .
	manualset3
109435	2	401978	13	NULL	NULL	0	NULL	GBD-CD2	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	It was constructed by rational truncation of GBD-CD2 , which harbors the second catalytic domain of DSR-E .
	manualset3
109436	3	401978	13	NULL	NULL	0	NULL	second catalytic domain 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	It was constructed by rational truncation of GBD-CD2 , which harbors the second catalytic domain of DSR-E .
	manualset3
109437	4	401978	13	NULL	NULL	0	NULL	DSR-E	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It was constructed by rational truncation of GBD-CD2 , which harbors the second catalytic domain of DSR-E .
	manualset3
109438	1	401979	13	NULL	NULL	0	NULL	E. coli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that E. coli and B. fragilis isolated from the normal intestinal flora of healthy individuals were susceptible to the bacteriocinogenic S. flexneri strains .
	manualset3
109439	2	401979	13	NULL	NULL	0	NULL	B. fragilis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that E. coli and B. fragilis isolated from the normal intestinal flora of healthy individuals were susceptible to the bacteriocinogenic S. flexneri strains .
	manualset3
109440	3	401979	13	NULL	NULL	0	NULL	normal intestinal flora	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that E. coli and B. fragilis isolated from the normal intestinal flora of healthy individuals were susceptible to the bacteriocinogenic S. flexneri strains .
	manualset3
109441	4	401979	13	NULL	NULL	0	NULL	healthy individuals 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that E. coli and B. fragilis isolated from the normal intestinal flora of healthy individuals were susceptible to the bacteriocinogenic S. flexneri strains .
	manualset3
109442	5	401979	13	NULL	NULL	0	NULL	bacteriocinogenic S. flexneri strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that E. coli and B. fragilis isolated from the normal intestinal flora of healthy individuals were susceptible to the bacteriocinogenic S. flexneri strains .
	manualset3
109443	1	401980	13	NULL	NULL	0	NULL	heavy CT regimen	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that a heavy CT regimen causing a severe toxicity did not always cause good results .
	manualset3
109444	2	401980	13	NULL	NULL	NULL	NULL	severe toxicity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was demonstrated that a heavy CT regimen causing a severe toxicity did not always cause good results .
	manualset3
109445	3	401980	13	NULL	NULL	0	NULL	good results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that a heavy CT regimen causing a severe toxicity did not always cause good results .
	manualset3
109446	1	401981	13	NULL	NULL	0	NULL	biofunctionalization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that biofunctionalization of planar microelectrode surface by covalently linking short peptides or fibronectin molecules could achieve strong or tight cell adhesion ( with an estimated averaged cell-to-substrate separation distance of 11-16 nm ) , which , in turn , improves the transduced electrical signal from IMA chips .
	manualset3
109447	2	401981	13	NULL	NULL	0	NULL	planar microelectrode surface	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that biofunctionalization of planar microelectrode surface by covalently linking short peptides or fibronectin molecules could achieve strong or tight cell adhesion ( with an estimated averaged cell-to-substrate separation distance of 11-16 nm ) , which , in turn , improves the transduced electrical signal from IMA chips .
	manualset3
109448	3	401981	13	NULL	NULL	0	NULL	short peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that biofunctionalization of planar microelectrode surface by covalently linking short peptides or fibronectin molecules could achieve strong or tight cell adhesion ( with an estimated averaged cell-to-substrate separation distance of 11-16 nm ) , which , in turn , improves the transduced electrical signal from IMA chips .
	manualset3
109449	4	401981	13	NULL	NULL	0	NULL	fibronectin molecules 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that biofunctionalization of planar microelectrode surface by covalently linking short peptides or fibronectin molecules could achieve strong or tight cell adhesion ( with an estimated averaged cell-to-substrate separation distance of 11-16 nm ) , which , in turn , improves the transduced electrical signal from IMA chips .
	manualset3
109450	5	401981	13	NULL	NULL	0	NULL	cell adhesion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that biofunctionalization of planar microelectrode surface by covalently linking short peptides or fibronectin molecules could achieve strong or tight cell adhesion ( with an estimated averaged cell-to-substrate separation distance of 11-16 nm ) , which , in turn , improves the transduced electrical signal from IMA chips .
	manualset3
109451	6	401981	13	NULL	NULL	0	NULL	cell-to-substrate separation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that biofunctionalization of planar microelectrode surface by covalently linking short peptides or fibronectin molecules could achieve strong or tight cell adhesion ( with an estimated averaged cell-to-substrate separation distance of 11-16 nm ) , which , in turn , improves the transduced electrical signal from IMA chips .
	manualset3
109452	7	401981	13	NULL	NULL	0	NULL	distance of 11-16 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that biofunctionalization of planar microelectrode surface by covalently linking short peptides or fibronectin molecules could achieve strong or tight cell adhesion ( with an estimated averaged cell-to-substrate separation distance of 11-16 nm ) , which , in turn , improves the transduced electrical signal from IMA chips .
	manualset3
109453	8	401981	13	NULL	NULL	0	NULL	electrical signal 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that biofunctionalization of planar microelectrode surface by covalently linking short peptides or fibronectin molecules could achieve strong or tight cell adhesion ( with an estimated averaged cell-to-substrate separation distance of 11-16 nm ) , which , in turn , improves the transduced electrical signal from IMA chips .
	manualset3
109454	9	401981	13	NULL	NULL	0	NULL	IMA chips	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that biofunctionalization of planar microelectrode surface by covalently linking short peptides or fibronectin molecules could achieve strong or tight cell adhesion ( with an estimated averaged cell-to-substrate separation distance of 11-16 nm ) , which , in turn , improves the transduced electrical signal from IMA chips .
	manualset3
109455	1	401982	13	NULL	NULL	0	NULL	sleep curtailment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that sleep curtailment may affect energy homeostasis of human organism with the effects on body weight increase through three different ways : appetite increase , prolongation of time for food intake and through decrease of energy expenditure .
	manualset3
109456	2	401982	13	NULL	NULL	0	NULL	energy homeostasis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that sleep curtailment may affect energy homeostasis of human organism with the effects on body weight increase through three different ways : appetite increase , prolongation of time for food intake and through decrease of energy expenditure .
	manualset3
109457	3	401982	13	NULL	NULL	0	NULL	human organism	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that sleep curtailment may affect energy homeostasis of human organism with the effects on body weight increase through three different ways : appetite increase , prolongation of time for food intake and through decrease of energy expenditure .
	manualset3
109458	4	401982	13	NULL	NULL	0	NULL	effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that sleep curtailment may affect energy homeostasis of human organism with the effects on body weight increase through three different ways : appetite increase , prolongation of time for food intake and through decrease of energy expenditure .
	manualset3
109459	5	401982	13	NULL	NULL	0	NULL	body weight increase	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that sleep curtailment may affect energy homeostasis of human organism with the effects on body weight increase through three different ways : appetite increase , prolongation of time for food intake and through decrease of energy expenditure .
	manualset3
109460	6	401982	13	NULL	NULL	0	NULL	three different ways	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that sleep curtailment may affect energy homeostasis of human organism with the effects on body weight increase through three different ways : appetite increase , prolongation of time for food intake and through decrease of energy expenditure .
	manualset3
109461	7	401982	13	NULL	NULL	0	NULL	appetite increase 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that sleep curtailment may affect energy homeostasis of human organism with the effects on body weight increase through three different ways : appetite increase , prolongation of time for food intake and through decrease of energy expenditure .
	manualset3
109462	8	401982	13	NULL	NULL	0	NULL	prolongation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that sleep curtailment may affect energy homeostasis of human organism with the effects on body weight increase through three different ways : appetite increase , prolongation of time for food intake and through decrease of energy expenditure .
	manualset3
109463	9	401982	13	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that sleep curtailment may affect energy homeostasis of human organism with the effects on body weight increase through three different ways : appetite increase , prolongation of time for food intake and through decrease of energy expenditure .
	manualset3
109464	10	401982	13	NULL	NULL	NULL	NULL	food intake	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was demonstrated that sleep curtailment may affect energy homeostasis of human organism with the effects on body weight increase through three different ways : appetite increase , prolongation of time for food intake and through decrease of energy expenditure .
	manualset3
109465	11	401982	13	NULL	NULL	0	NULL	energy expenditure	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that sleep curtailment may affect energy homeostasis of human organism with the effects on body weight increase through three different ways : appetite increase , prolongation of time for food intake and through decrease of energy expenditure .
	manualset3
112984	12	401982	13	NULL	NULL	0	NULL	decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that sleep curtailment may affect energy homeostasis of human organism with the effects on body weight increase through three different ways : appetite increase , prolongation of time for food intake and through decrease of energy expenditure .
	manualset3
109466	1	401983	13	NULL	NULL	0	NULL	9 , 10-Diphenylanthracene ( DPA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	9 , 10-Diphenylanthracene ( DPA ) , a well-studied organic chromophore ( Phi ( fl ) = 0.98 ) that exhibits electroluminescence , has been covalently bound through 2 - ( ethylthio ) ethylamido linkers to the carboxylic acid groups of short , soluble single-walled carbon nanotubes ( sSWNTs ) of 1 microm average length , and the resulting DPA-functionalised sSWNT ( DPA - sSWNT ) macromolecular adducts ( 4.6 wt % DPA content ) characterised by solution ( 1 ) H NMR , Raman and IR spectroscopy and thermogravimetric analysis .
	manualset3
109467	2	401983	13	NULL	NULL	0	NULL	organic chromophore 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	9 , 10-Diphenylanthracene ( DPA ) , a well-studied organic chromophore ( Phi ( fl ) = 0.98 ) that exhibits electroluminescence , has been covalently bound through 2 - ( ethylthio ) ethylamido linkers to the carboxylic acid groups of short , soluble single-walled carbon nanotubes ( sSWNTs ) of 1 microm average length , and the resulting DPA-functionalised sSWNT ( DPA - sSWNT ) macromolecular adducts ( 4.6 wt % DPA content ) characterised by solution ( 1 ) H NMR , Raman and IR spectroscopy and thermogravimetric analysis .
	manualset3
109468	3	401983	13	NULL	NULL	0	NULL	Phi ( fl ) = 0.98	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	9 , 10-Diphenylanthracene ( DPA ) , a well-studied organic chromophore ( Phi ( fl ) = 0.98 ) that exhibits electroluminescence , has been covalently bound through 2 - ( ethylthio ) ethylamido linkers to the carboxylic acid groups of short , soluble single-walled carbon nanotubes ( sSWNTs ) of 1 microm average length , and the resulting DPA-functionalised sSWNT ( DPA - sSWNT ) macromolecular adducts ( 4.6 wt % DPA content ) characterised by solution ( 1 ) H NMR , Raman and IR spectroscopy and thermogravimetric analysis .
	manualset3
109469	4	401983	13	NULL	NULL	0	NULL	electroluminescence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	9 , 10-Diphenylanthracene ( DPA ) , a well-studied organic chromophore ( Phi ( fl ) = 0.98 ) that exhibits electroluminescence , has been covalently bound through 2 - ( ethylthio ) ethylamido linkers to the carboxylic acid groups of short , soluble single-walled carbon nanotubes ( sSWNTs ) of 1 microm average length , and the resulting DPA-functionalised sSWNT ( DPA - sSWNT ) macromolecular adducts ( 4.6 wt % DPA content ) characterised by solution ( 1 ) H NMR , Raman and IR spectroscopy and thermogravimetric analysis .
	manualset3
109470	5	401983	13	NULL	NULL	0	NULL	 2 - ( ethylthio ) ethylamido linkers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	9 , 10-Diphenylanthracene ( DPA ) , a well-studied organic chromophore ( Phi ( fl ) = 0.98 ) that exhibits electroluminescence , has been covalently bound through 2 - ( ethylthio ) ethylamido linkers to the carboxylic acid groups of short , soluble single-walled carbon nanotubes ( sSWNTs ) of 1 microm average length , and the resulting DPA-functionalised sSWNT ( DPA - sSWNT ) macromolecular adducts ( 4.6 wt % DPA content ) characterised by solution ( 1 ) H NMR , Raman and IR spectroscopy and thermogravimetric analysis .
	manualset3
109471	6	401983	13	NULL	NULL	0	NULL	carboxylic acid groups 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	9 , 10-Diphenylanthracene ( DPA ) , a well-studied organic chromophore ( Phi ( fl ) = 0.98 ) that exhibits electroluminescence , has been covalently bound through 2 - ( ethylthio ) ethylamido linkers to the carboxylic acid groups of short , soluble single-walled carbon nanotubes ( sSWNTs ) of 1 microm average length , and the resulting DPA-functionalised sSWNT ( DPA - sSWNT ) macromolecular adducts ( 4.6 wt % DPA content ) characterised by solution ( 1 ) H NMR , Raman and IR spectroscopy and thermogravimetric analysis .
	manualset3
109472	7	401983	13	NULL	NULL	0	NULL	short , soluble single-walled carbon nanotubes ( sSWNTs )	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	9 , 10-Diphenylanthracene ( DPA ) , a well-studied organic chromophore ( Phi ( fl ) = 0.98 ) that exhibits electroluminescence , has been covalently bound through 2 - ( ethylthio ) ethylamido linkers to the carboxylic acid groups of short , soluble single-walled carbon nanotubes ( sSWNTs ) of 1 microm average length , and the resulting DPA-functionalised sSWNT ( DPA - sSWNT ) macromolecular adducts ( 4.6 wt % DPA content ) characterised by solution ( 1 ) H NMR , Raman and IR spectroscopy and thermogravimetric analysis .
	manualset3
109473	8	401983	13	NULL	NULL	0	NULL	1 microm average length	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	9 , 10-Diphenylanthracene ( DPA ) , a well-studied organic chromophore ( Phi ( fl ) = 0.98 ) that exhibits electroluminescence , has been covalently bound through 2 - ( ethylthio ) ethylamido linkers to the carboxylic acid groups of short , soluble single-walled carbon nanotubes ( sSWNTs ) of 1 microm average length , and the resulting DPA-functionalised sSWNT ( DPA - sSWNT ) macromolecular adducts ( 4.6 wt % DPA content ) characterised by solution ( 1 ) H NMR , Raman and IR spectroscopy and thermogravimetric analysis .
	manualset3
109474	9	401983	13	NULL	NULL	0	NULL	DPA-functionalised sSWNT ( DPA - sSWNT )	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	9 , 10-Diphenylanthracene ( DPA ) , a well-studied organic chromophore ( Phi ( fl ) = 0.98 ) that exhibits electroluminescence , has been covalently bound through 2 - ( ethylthio ) ethylamido linkers to the carboxylic acid groups of short , soluble single-walled carbon nanotubes ( sSWNTs ) of 1 microm average length , and the resulting DPA-functionalised sSWNT ( DPA - sSWNT ) macromolecular adducts ( 4.6 wt % DPA content ) characterised by solution ( 1 ) H NMR , Raman and IR spectroscopy and thermogravimetric analysis .
	manualset3
109475	10	401983	13	NULL	NULL	0	NULL	macromolecular adducts 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	9 , 10-Diphenylanthracene ( DPA ) , a well-studied organic chromophore ( Phi ( fl ) = 0.98 ) that exhibits electroluminescence , has been covalently bound through 2 - ( ethylthio ) ethylamido linkers to the carboxylic acid groups of short , soluble single-walled carbon nanotubes ( sSWNTs ) of 1 microm average length , and the resulting DPA-functionalised sSWNT ( DPA - sSWNT ) macromolecular adducts ( 4.6 wt % DPA content ) characterised by solution ( 1 ) H NMR , Raman and IR spectroscopy and thermogravimetric analysis .
	manualset3
109476	11	401983	13	NULL	NULL	0	NULL	4.6 wt % DPA content	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	9 , 10-Diphenylanthracene ( DPA ) , a well-studied organic chromophore ( Phi ( fl ) = 0.98 ) that exhibits electroluminescence , has been covalently bound through 2 - ( ethylthio ) ethylamido linkers to the carboxylic acid groups of short , soluble single-walled carbon nanotubes ( sSWNTs ) of 1 microm average length , and the resulting DPA-functionalised sSWNT ( DPA - sSWNT ) macromolecular adducts ( 4.6 wt % DPA content ) characterised by solution ( 1 ) H NMR , Raman and IR spectroscopy and thermogravimetric analysis .
	manualset3
109508	12	401983	13	NULL	NULL	0	NULL	solution ( 1 ) H NMR 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	9 , 10-Diphenylanthracene ( DPA ) , a well-studied organic chromophore ( Phi ( fl ) = 0.98 ) that exhibits electroluminescence , has been covalently bound through 2 - ( ethylthio ) ethylamido linkers to the carboxylic acid groups of short , soluble single-walled carbon nanotubes ( sSWNTs ) of 1 microm average length , and the resulting DPA-functionalised sSWNT ( DPA - sSWNT ) macromolecular adducts ( 4.6 wt % DPA content ) characterised by solution ( 1 ) H NMR , Raman and IR spectroscopy and thermogravimetric analysis .
	manualset3
109509	13	401983	13	NULL	NULL	0	NULL	Raman spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	9 , 10-Diphenylanthracene ( DPA ) , a well-studied organic chromophore ( Phi ( fl ) = 0.98 ) that exhibits electroluminescence , has been covalently bound through 2 - ( ethylthio ) ethylamido linkers to the carboxylic acid groups of short , soluble single-walled carbon nanotubes ( sSWNTs ) of 1 microm average length , and the resulting DPA-functionalised sSWNT ( DPA - sSWNT ) macromolecular adducts ( 4.6 wt % DPA content ) characterised by solution ( 1 ) H NMR , Raman and IR spectroscopy and thermogravimetric analysis .
	manualset3
109510	14	401983	13	NULL	NULL	0	NULL	IR spectroscopy 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	9 , 10-Diphenylanthracene ( DPA ) , a well-studied organic chromophore ( Phi ( fl ) = 0.98 ) that exhibits electroluminescence , has been covalently bound through 2 - ( ethylthio ) ethylamido linkers to the carboxylic acid groups of short , soluble single-walled carbon nanotubes ( sSWNTs ) of 1 microm average length , and the resulting DPA-functionalised sSWNT ( DPA - sSWNT ) macromolecular adducts ( 4.6 wt % DPA content ) characterised by solution ( 1 ) H NMR , Raman and IR spectroscopy and thermogravimetric analysis .
	manualset3
109511	15	401983	13	NULL	NULL	0	NULL	 thermogravimetric analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	9 , 10-Diphenylanthracene ( DPA ) , a well-studied organic chromophore ( Phi ( fl ) = 0.98 ) that exhibits electroluminescence , has been covalently bound through 2 - ( ethylthio ) ethylamido linkers to the carboxylic acid groups of short , soluble single-walled carbon nanotubes ( sSWNTs ) of 1 microm average length , and the resulting DPA-functionalised sSWNT ( DPA - sSWNT ) macromolecular adducts ( 4.6 wt % DPA content ) characterised by solution ( 1 ) H NMR , Raman and IR spectroscopy and thermogravimetric analysis .
	manualset3
109498	1	401984	13	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that the development of experimental avitaminosis A in chicks led to secondary zinc deficiency .
	manualset3
109499	2	401984	13	NULL	NULL	0	NULL	experimental avitaminosis A	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that the development of experimental avitaminosis A in chicks led to secondary zinc deficiency .
	manualset3
109500	3	401984	13	NULL	NULL	0	NULL	chicks	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that the development of experimental avitaminosis A in chicks led to secondary zinc deficiency .
	manualset3
109501	4	401984	13	NULL	NULL	0	NULL	secondary zinc deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that the development of experimental avitaminosis A in chicks led to secondary zinc deficiency .
	manualset3
109526	1	401985	13	NULL	NULL	0	NULL	denaturation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that under denaturation the DNA filaments do not break apart completely .
	manualset3
109527	2	401985	13	NULL	NULL	0	NULL	DNA filaments 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It was demonstrated that under denaturation the DNA filaments do not break apart completely .
	manualset3
109528	1	401986	13	NULL	NULL	NULL	NULL	differential diagnosis	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was difficult to make a differential diagnosis because prominent CT formed a bridge-like shape in this case .
	manualset3
109529	2	401986	13	NULL	NULL	0	NULL	CT	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It was difficult to make a differential diagnosis because prominent CT formed a bridge-like shape in this case .
	manualset3
109530	3	401986	13	NULL	NULL	0	NULL	bridge-like shape	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It was difficult to make a differential diagnosis because prominent CT formed a bridge-like shape in this case .
	manualset3
109531	4	401986	13	NULL	NULL	0	NULL	case	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	It was difficult to make a differential diagnosis because prominent CT formed a bridge-like shape in this case .
	manualset3
109536	1	401987	13	NULL	NULL	0	NULL	aerobic conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	It was effective under both aerobic and anaerobic conditions , while similar testing of the desnitro niridazole produced consistently negative results .
	manualset3
109537	2	401987	13	NULL	NULL	0	NULL	anaerobic conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	It was effective under both aerobic and anaerobic conditions , while similar testing of the desnitro niridazole produced consistently negative results .
	manualset3
109538	3	401987	13	NULL	NULL	0	NULL	testing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	It was effective under both aerobic and anaerobic conditions , while similar testing of the desnitro niridazole produced consistently negative results .
	manualset3
109539	4	401987	13	NULL	NULL	0	NULL	desnitro niridazole 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was effective under both aerobic and anaerobic conditions , while similar testing of the desnitro niridazole produced consistently negative results .
	manualset3
109608	1	401988	13	NULL	NULL	0	NULL	noni fruit juice	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	It was elucidated that the noni fruit juice inhibitory effect on XO enzymes is the mechanism by which noni ameliorates gout and gout-like diseases .
	manualset3
109609	2	401988	13	NULL	NULL	0	NULL	inhibitory effect 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was elucidated that the noni fruit juice inhibitory effect on XO enzymes is the mechanism by which noni ameliorates gout and gout-like diseases .
	manualset3
109610	3	401988	13	NULL	NULL	0	NULL	XO enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It was elucidated that the noni fruit juice inhibitory effect on XO enzymes is the mechanism by which noni ameliorates gout and gout-like diseases .
	manualset3
109611	4	401988	13	NULL	NULL	0	NULL	mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was elucidated that the noni fruit juice inhibitory effect on XO enzymes is the mechanism by which noni ameliorates gout and gout-like diseases .
	manualset3
109612	5	401988	13	NULL	NULL	0	NULL	noni	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	It was elucidated that the noni fruit juice inhibitory effect on XO enzymes is the mechanism by which noni ameliorates gout and gout-like diseases .
	manualset3
109613	6	401988	13	NULL	NULL	0	NULL	gout	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It was elucidated that the noni fruit juice inhibitory effect on XO enzymes is the mechanism by which noni ameliorates gout and gout-like diseases .
	manualset3
109614	7	401988	13	NULL	NULL	0	NULL	gout-like diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It was elucidated that the noni fruit juice inhibitory effect on XO enzymes is the mechanism by which noni ameliorates gout and gout-like diseases .
	manualset3
109615	1	401989	13	NULL	NULL	0	NULL	drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	It was established that drug uptake was significantly more rapid and quantitatively greater in drug-sensitive parasites .
	manualset3
109616	2	401989	13	NULL	NULL	NULL	NULL	uptake	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was established that drug uptake was significantly more rapid and quantitatively greater in drug-sensitive parasites .
	manualset3
109617	3	401989	13	NULL	NULL	0	NULL	drug-sensitive parasites	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It was established that drug uptake was significantly more rapid and quantitatively greater in drug-sensitive parasites .
	manualset3
109618	1	401990	13	NULL	NULL	0	NULL	variation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	It was established that the variation in the amounts of enderpines in the myocardium , hypothalamus , and adrenals of humans who had died suddenly is not accidental but is determined to a certain extent by such factors as type of tissue and age .
	manualset3
109619	2	401990	13	NULL	NULL	0	NULL	amounts	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was established that the variation in the amounts of enderpines in the myocardium , hypothalamus , and adrenals of humans who had died suddenly is not accidental but is determined to a certain extent by such factors as type of tissue and age .
	manualset3
109620	3	401990	13	NULL	NULL	0	NULL	enderpines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was established that the variation in the amounts of enderpines in the myocardium , hypothalamus , and adrenals of humans who had died suddenly is not accidental but is determined to a certain extent by such factors as type of tissue and age .
	manualset3
109621	4	401990	13	NULL	NULL	0	NULL	myocardium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It was established that the variation in the amounts of enderpines in the myocardium , hypothalamus , and adrenals of humans who had died suddenly is not accidental but is determined to a certain extent by such factors as type of tissue and age .
	manualset3
109622	5	401990	13	NULL	NULL	0	NULL	hypothalamus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It was established that the variation in the amounts of enderpines in the myocardium , hypothalamus , and adrenals of humans who had died suddenly is not accidental but is determined to a certain extent by such factors as type of tissue and age .
	manualset3
109623	6	401990	13	NULL	NULL	0	NULL	adrenals 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It was established that the variation in the amounts of enderpines in the myocardium , hypothalamus , and adrenals of humans who had died suddenly is not accidental but is determined to a certain extent by such factors as type of tissue and age .
	manualset3
109625	7	401990	13	NULL	NULL	0	NULL	humans	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It was established that the variation in the amounts of enderpines in the myocardium , hypothalamus , and adrenals of humans who had died suddenly is not accidental but is determined to a certain extent by such factors as type of tissue and age .
	manualset3
109626	8	401990	13	NULL	NULL	0	NULL	extent	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was established that the variation in the amounts of enderpines in the myocardium , hypothalamus , and adrenals of humans who had died suddenly is not accidental but is determined to a certain extent by such factors as type of tissue and age .
	manualset3
109627	9	401990	13	NULL	NULL	0	NULL	factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was established that the variation in the amounts of enderpines in the myocardium , hypothalamus , and adrenals of humans who had died suddenly is not accidental but is determined to a certain extent by such factors as type of tissue and age .
	manualset3
109628	10	401990	13	NULL	NULL	NULL	NULL	type of tissue 	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was established that the variation in the amounts of enderpines in the myocardium , hypothalamus , and adrenals of humans who had died suddenly is not accidental but is determined to a certain extent by such factors as type of tissue and age .
	manualset3
109629	11	401990	13	NULL	NULL	0	NULL	age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was established that the variation in the amounts of enderpines in the myocardium , hypothalamus , and adrenals of humans who had died suddenly is not accidental but is determined to a certain extent by such factors as type of tissue and age .
	manualset3
109630	1	401991	13	NULL	NULL	0	NULL	9 , 67 ( 2002 ) ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	9 , 67 ( 2002 ) ) , which involves the dynamics of the mRNA , given protein and metabolite concentrations .
	manualset3
109631	2	401991	13	NULL	NULL	0	NULL	dynamics	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	9 , 67 ( 2002 ) ) , which involves the dynamics of the mRNA , given protein and metabolite concentrations .
	manualset3
109632	3	401991	13	NULL	NULL	0	NULL	mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	9 , 67 ( 2002 ) ) , which involves the dynamics of the mRNA , given protein and metabolite concentrations .
	manualset3
109633	4	401991	13	NULL	NULL	0	NULL	protein concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	9 , 67 ( 2002 ) ) , which involves the dynamics of the mRNA , given protein and metabolite concentrations .
	manualset3
109634	5	401991	13	NULL	NULL	0	NULL	metabolite concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	9 , 67 ( 2002 ) ) , which involves the dynamics of the mRNA , given protein and metabolite concentrations .
	manualset3
109635	1	401992	13	NULL	NULL	0	NULL	NO2 - release 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that NO2 - release was dependent on the nature of thiol .
	manualset3
109636	2	401992	13	NULL	NULL	0	NULL	thiol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that NO2 - release was dependent on the nature of thiol .
	manualset3
109637	1	401993	13	NULL	NULL	0	NULL	PVA/PVP-stabilized silver nanocomposite film	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that PVA/PVP-stabilized silver nanocomposite film revealed the presence of well-dispersed and spherical silver nanoparticles with an average diameter of 30nm , while the particle sizes were reduced as the PVP percentage increased .
	manualset3
109638	2	401993	13	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that PVA/PVP-stabilized silver nanocomposite film revealed the presence of well-dispersed and spherical silver nanoparticles with an average diameter of 30nm , while the particle sizes were reduced as the PVP percentage increased .
	manualset3
109639	3	401993	13	NULL	NULL	0	NULL	silver nanoparticles	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that PVA/PVP-stabilized silver nanocomposite film revealed the presence of well-dispersed and spherical silver nanoparticles with an average diameter of 30nm , while the particle sizes were reduced as the PVP percentage increased .
	manualset3
109640	4	401993	13	NULL	NULL	0	NULL	average diameter	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that PVA/PVP-stabilized silver nanocomposite film revealed the presence of well-dispersed and spherical silver nanoparticles with an average diameter of 30nm , while the particle sizes were reduced as the PVP percentage increased .
	manualset3
109641	5	401993	13	NULL	NULL	0	NULL	30nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that PVA/PVP-stabilized silver nanocomposite film revealed the presence of well-dispersed and spherical silver nanoparticles with an average diameter of 30nm , while the particle sizes were reduced as the PVP percentage increased .
	manualset3
109642	6	401993	13	NULL	NULL	0	NULL	particle sizes	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that PVA/PVP-stabilized silver nanocomposite film revealed the presence of well-dispersed and spherical silver nanoparticles with an average diameter of 30nm , while the particle sizes were reduced as the PVP percentage increased .
	manualset3
109643	7	401993	13	NULL	NULL	0	NULL	PVP percentage	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that PVA/PVP-stabilized silver nanocomposite film revealed the presence of well-dispersed and spherical silver nanoparticles with an average diameter of 30nm , while the particle sizes were reduced as the PVP percentage increased .
	manualset3
109644	1	401994	13	NULL	NULL	0	NULL	T. cutaneum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that T. cutaneum gave a greater response to glucose , whereas B. licheniformis gave a better response to glutamic acid .
	manualset3
109645	2	401994	13	NULL	NULL	0	NULL	response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that T. cutaneum gave a greater response to glucose , whereas B. licheniformis gave a better response to glutamic acid .
	manualset3
109646	3	401994	13	NULL	NULL	0	NULL	glucose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that T. cutaneum gave a greater response to glucose , whereas B. licheniformis gave a better response to glutamic acid .
	manualset3
109647	4	401994	13	NULL	NULL	0	NULL	 B. licheniformis 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that T. cutaneum gave a greater response to glucose , whereas B. licheniformis gave a better response to glutamic acid .
	manualset3
109648	5	401994	13	NULL	NULL	0	NULL	response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that T. cutaneum gave a greater response to glucose , whereas B. licheniformis gave a better response to glutamic acid .
	manualset3
109649	6	401994	13	NULL	NULL	0	NULL	glutamic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that T. cutaneum gave a greater response to glucose , whereas B. licheniformis gave a better response to glutamic acid .
	manualset3
109650	1	401995	13	NULL	NULL	0	NULL	non-linear model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that a non-linear model is slightly better than linear model in terms of percentage prediction errors .
	manualset3
109651	2	401995	13	NULL	NULL	0	NULL	linear model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that a non-linear model is slightly better than linear model in terms of percentage prediction errors .
	manualset3
109652	3	401995	13	NULL	NULL	0	NULL	terms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that a non-linear model is slightly better than linear model in terms of percentage prediction errors .
	manualset3
109653	4	401995	13	NULL	NULL	0	NULL	percentage prediction errors	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that a non-linear model is slightly better than linear model in terms of percentage prediction errors .
	manualset3
109654	1	401996	13	NULL	NULL	0	NULL	 calcium oxalate dihydrate calculi	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that calcium oxalate dihydrate calculi decreased with age , but only in men .
	manualset3
109655	2	401996	13	NULL	NULL	0	NULL	age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that calcium oxalate dihydrate calculi decreased with age , but only in men .
	manualset3
109656	3	401996	13	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that calcium oxalate dihydrate calculi decreased with age , but only in men .
	manualset3
109657	1	401997	13	NULL	NULL	0	NULL	diperiodatocuprate ( III ) ( K ( 5 ) ( Cu ( HIO ( 6 ) ) ( 2 ) ) , DPC )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that diperiodatocuprate ( III ) ( K ( 5 ) ( Cu ( HIO ( 6 ) ) ( 2 ) ) , DPC ) , a transition metal chelate at unstable high oxidation state , could effectively enhance the reaction between luminol-type compound and hydrogen peroxide , to produce very strong CL signal .
	manualset3
109706	2	401997	13	NULL	NULL	0	NULL	transition metal chelate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that diperiodatocuprate ( III ) ( K ( 5 ) ( Cu ( HIO ( 6 ) ) ( 2 ) ) , DPC ) , a transition metal chelate at unstable high oxidation state , could effectively enhance the reaction between luminol-type compound and hydrogen peroxide , to produce very strong CL signal .
	manualset3
109707	3	401997	13	NULL	NULL	0	NULL	oxidation state 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that diperiodatocuprate ( III ) ( K ( 5 ) ( Cu ( HIO ( 6 ) ) ( 2 ) ) , DPC ) , a transition metal chelate at unstable high oxidation state , could effectively enhance the reaction between luminol-type compound and hydrogen peroxide , to produce very strong CL signal .
	manualset3
109708	4	401997	13	NULL	NULL	0	NULL	reaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that diperiodatocuprate ( III ) ( K ( 5 ) ( Cu ( HIO ( 6 ) ) ( 2 ) ) , DPC ) , a transition metal chelate at unstable high oxidation state , could effectively enhance the reaction between luminol-type compound and hydrogen peroxide , to produce very strong CL signal .
	manualset3
109709	5	401997	13	NULL	NULL	0	NULL	luminol-type compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that diperiodatocuprate ( III ) ( K ( 5 ) ( Cu ( HIO ( 6 ) ) ( 2 ) ) , DPC ) , a transition metal chelate at unstable high oxidation state , could effectively enhance the reaction between luminol-type compound and hydrogen peroxide , to produce very strong CL signal .
	manualset3
109710	6	401997	13	NULL	NULL	0	NULL	hydrogen peroxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that diperiodatocuprate ( III ) ( K ( 5 ) ( Cu ( HIO ( 6 ) ) ( 2 ) ) , DPC ) , a transition metal chelate at unstable high oxidation state , could effectively enhance the reaction between luminol-type compound and hydrogen peroxide , to produce very strong CL signal .
	manualset3
109711	7	401997	13	NULL	NULL	0	NULL	CL signal 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that diperiodatocuprate ( III ) ( K ( 5 ) ( Cu ( HIO ( 6 ) ) ( 2 ) ) , DPC ) , a transition metal chelate at unstable high oxidation state , could effectively enhance the reaction between luminol-type compound and hydrogen peroxide , to produce very strong CL signal .
	manualset3
109712	1	401998	13	NULL	NULL	0	NULL	90 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	90 % of the population is of European descent , largely as a result of high rates of immigration during the 1880s-1930s from countries such as Spain and Italy .
	manualset3
109789	2	401998	13	NULL	NULL	0	NULL	population 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	90 % of the population is of European descent , largely as a result of high rates of immigration during the 1880s-1930s from countries such as Spain and Italy .
	manualset3
109790	3	401998	13	NULL	NULL	0	NULL	European descent	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	90 % of the population is of European descent , largely as a result of high rates of immigration during the 1880s-1930s from countries such as Spain and Italy .
	manualset3
109791	4	401998	13	NULL	NULL	0	NULL	result	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	90 % of the population is of European descent , largely as a result of high rates of immigration during the 1880s-1930s from countries such as Spain and Italy .
	manualset3
109792	5	401998	13	NULL	NULL	0	NULL	high rates	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	90 % of the population is of European descent , largely as a result of high rates of immigration during the 1880s-1930s from countries such as Spain and Italy .
	manualset3
109793	6	401998	13	NULL	NULL	0	NULL	immigration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	90 % of the population is of European descent , largely as a result of high rates of immigration during the 1880s-1930s from countries such as Spain and Italy .
	manualset3
109794	7	401998	13	NULL	NULL	0	NULL	1880s-1930s	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	90 % of the population is of European descent , largely as a result of high rates of immigration during the 1880s-1930s from countries such as Spain and Italy .
	manualset3
109795	8	401998	13	NULL	NULL	0	NULL	countries	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	90 % of the population is of European descent , largely as a result of high rates of immigration during the 1880s-1930s from countries such as Spain and Italy .
	manualset3
109796	9	401998	13	NULL	NULL	0	NULL	Spain	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	90 % of the population is of European descent , largely as a result of high rates of immigration during the 1880s-1930s from countries such as Spain and Italy .
	manualset3
109797	10	401998	13	NULL	NULL	0	NULL	Italy	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	90 % of the population is of European descent , largely as a result of high rates of immigration during the 1880s-1930s from countries such as Spain and Italy .
	manualset3
109798	1	401999	13	NULL	NULL	0	NULL	exhaustive washing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that even after exhaustive washing with aqueous base the purified SWNTs contain carboxylic acid groups in sufficient quantity to prepare high quality soluble SWNT materials by covalent functionalization with octadecylamine .
	manualset3
109799	2	401999	13	NULL	NULL	0	NULL	aqueous base	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that even after exhaustive washing with aqueous base the purified SWNTs contain carboxylic acid groups in sufficient quantity to prepare high quality soluble SWNT materials by covalent functionalization with octadecylamine .
	manualset3
109800	3	401999	13	NULL	NULL	0	NULL	SWNTs	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that even after exhaustive washing with aqueous base the purified SWNTs contain carboxylic acid groups in sufficient quantity to prepare high quality soluble SWNT materials by covalent functionalization with octadecylamine .
	manualset3
109801	4	401999	13	NULL	NULL	0	NULL	carboxylic acid groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that even after exhaustive washing with aqueous base the purified SWNTs contain carboxylic acid groups in sufficient quantity to prepare high quality soluble SWNT materials by covalent functionalization with octadecylamine .
	manualset3
109802	5	401999	13	NULL	NULL	0	NULL	quantity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that even after exhaustive washing with aqueous base the purified SWNTs contain carboxylic acid groups in sufficient quantity to prepare high quality soluble SWNT materials by covalent functionalization with octadecylamine .
	manualset3
109803	6	401999	13	NULL	NULL	0	NULL	quality	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that even after exhaustive washing with aqueous base the purified SWNTs contain carboxylic acid groups in sufficient quantity to prepare high quality soluble SWNT materials by covalent functionalization with octadecylamine .
	manualset3
109804	7	401999	13	NULL	NULL	0	NULL	soluble SWNT materials	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that even after exhaustive washing with aqueous base the purified SWNTs contain carboxylic acid groups in sufficient quantity to prepare high quality soluble SWNT materials by covalent functionalization with octadecylamine .
	manualset3
109805	8	401999	13	NULL	NULL	0	NULL	covalent functionalization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that even after exhaustive washing with aqueous base the purified SWNTs contain carboxylic acid groups in sufficient quantity to prepare high quality soluble SWNT materials by covalent functionalization with octadecylamine .
	manualset3
109806	9	401999	13	NULL	NULL	0	NULL	octadecylamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that even after exhaustive washing with aqueous base the purified SWNTs contain carboxylic acid groups in sufficient quantity to prepare high quality soluble SWNT materials by covalent functionalization with octadecylamine .
	manualset3
109807	1	402000	13	NULL	NULL	NULL	NULL	21 , 493  	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was found that from the 21 , 493 gene-probes detected throughout development , 302 protein-coding transcripts were upregulated during the initiation of synapse formation .
	manualset3
109808	3	402000	13	NULL	NULL	NULL	NULL	development	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was found that from the 21 , 493 gene-probes detected throughout development , 302 protein-coding transcripts were upregulated during the initiation of synapse formation .
	manualset3
109809	4	402000	13	NULL	NULL	NULL	NULL	302 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was found that from the 21 , 493 gene-probes detected throughout development , 302 protein-coding transcripts were upregulated during the initiation of synapse formation .
	manualset3
109810	2	402000	13	NULL	NULL	0	NULL	gene-probes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that from the 21 , 493 gene-probes detected throughout development , 302 protein-coding transcripts were upregulated during the initiation of synapse formation .
	manualset3
109811	5	402000	13	NULL	NULL	0	NULL	protein-coding transcripts 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that from the 21 , 493 gene-probes detected throughout development , 302 protein-coding transcripts were upregulated during the initiation of synapse formation .
	manualset3
109812	6	402000	13	NULL	NULL	0	NULL	initiation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that from the 21 , 493 gene-probes detected throughout development , 302 protein-coding transcripts were upregulated during the initiation of synapse formation .
	manualset3
109813	7	402000	13	NULL	NULL	NULL	NULL	synapse formation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was found that from the 21 , 493 gene-probes detected throughout development , 302 protein-coding transcripts were upregulated during the initiation of synapse formation .
	manualset3
109814	1	402001	13	NULL	NULL	0	NULL	forefoot	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that in normal barefoot walking the forefoot carried a total load of the order of three times that of the heel .
	manualset3
109816	3	402001	13	NULL	NULL	0	NULL	order	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that in normal barefoot walking the forefoot carried a total load of the order of three times that of the heel .
	manualset3
109817	4	402001	13	NULL	NULL	0	NULL	three times 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that in normal barefoot walking the forefoot carried a total load of the order of three times that of the heel .
	manualset3
109818	5	402001	13	NULL	NULL	0	NULL	heel	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that in normal barefoot walking the forefoot carried a total load of the order of three times that of the heel .
	manualset3
109815	1	402002	13	NULL	NULL	NULL	NULL	water	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was found that in water MS2 phage is significantly more sensitive to ionizing radiation than Escherichia coli .
	manualset3
109819	2	402002	13	NULL	NULL	0	NULL	MS2 phage	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that in water MS2 phage is significantly more sensitive to ionizing radiation than Escherichia coli .
	manualset3
109820	3	402002	13	NULL	NULL	0	NULL	radiation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that in water MS2 phage is significantly more sensitive to ionizing radiation than Escherichia coli .
	manualset3
109821	4	402002	13	NULL	NULL	0	NULL	Escherichia coli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that in water MS2 phage is significantly more sensitive to ionizing radiation than Escherichia coli .
	manualset3
109822	1	402003	13	NULL	NULL	0	NULL	inattention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that left-sided inattention predicted transmission of the 10-repeat allele from parents to probands and was associated with the severity of ADHD symptomatology .
	manualset3
109823	2	402003	13	NULL	NULL	0	NULL	transmission	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that left-sided inattention predicted transmission of the 10-repeat allele from parents to probands and was associated with the severity of ADHD symptomatology .
	manualset3
109824	3	402003	13	NULL	NULL	0	NULL	10-repeat allele	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that left-sided inattention predicted transmission of the 10-repeat allele from parents to probands and was associated with the severity of ADHD symptomatology .
	manualset3
109825	4	402003	13	NULL	NULL	0	NULL	parents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that left-sided inattention predicted transmission of the 10-repeat allele from parents to probands and was associated with the severity of ADHD symptomatology .
	manualset3
109826	5	402003	13	NULL	NULL	0	NULL	probands	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that left-sided inattention predicted transmission of the 10-repeat allele from parents to probands and was associated with the severity of ADHD symptomatology .
	manualset3
109827	6	402003	13	NULL	NULL	0	NULL	severity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that left-sided inattention predicted transmission of the 10-repeat allele from parents to probands and was associated with the severity of ADHD symptomatology .
	manualset3
109828	7	402003	13	NULL	NULL	0	NULL	ADHD symptomatology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that left-sided inattention predicted transmission of the 10-repeat allele from parents to probands and was associated with the severity of ADHD symptomatology .
	manualset3
109829	1	402004	13	NULL	NULL	0	NULL	content 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that the content of s-SWCNTs in the samples was highly sensitive to the amount of oxygen introduced .
	manualset3
109830	2	402004	13	NULL	NULL	0	NULL	s-SWCNTs	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that the content of s-SWCNTs in the samples was highly sensitive to the amount of oxygen introduced .
	manualset3
109831	3	402004	13	NULL	NULL	0	NULL	samples	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that the content of s-SWCNTs in the samples was highly sensitive to the amount of oxygen introduced .
	manualset3
109832	4	402004	13	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that the content of s-SWCNTs in the samples was highly sensitive to the amount of oxygen introduced .
	manualset3
109833	5	402004	13	NULL	NULL	0	NULL	oxygen	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that the content of s-SWCNTs in the samples was highly sensitive to the amount of oxygen introduced .
	manualset3
109834	1	402005	13	NULL	NULL	NULL	NULL	intercellular matrix 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was found that the intercellular matrix of Bacillus subtilis 271 mainly consists of alpha-1 , 4 - glucan ( 65 % of dry matter ) , branched at some C-3 residues of the polymeric chain , and poly-D-glutamic acid ( 19 % of dry matter ) .
	manualset3
109835	2	402005	13	NULL	NULL	0	NULL	Bacillus subtilis 271	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that the intercellular matrix of Bacillus subtilis 271 mainly consists of alpha-1 , 4 - glucan ( 65 % of dry matter ) , branched at some C-3 residues of the polymeric chain , and poly-D-glutamic acid ( 19 % of dry matter ) .
	manualset3
109836	3	402005	13	NULL	NULL	0	NULL	alpha-1 , 4 - glucan 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that the intercellular matrix of Bacillus subtilis 271 mainly consists of alpha-1 , 4 - glucan ( 65 % of dry matter ) , branched at some C-3 residues of the polymeric chain , and poly-D-glutamic acid ( 19 % of dry matter ) .
	manualset3
109837	4	402005	13	NULL	NULL	0	NULL	65 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that the intercellular matrix of Bacillus subtilis 271 mainly consists of alpha-1 , 4 - glucan ( 65 % of dry matter ) , branched at some C-3 residues of the polymeric chain , and poly-D-glutamic acid ( 19 % of dry matter ) .
	manualset3
109838	5	402005	13	NULL	NULL	0	NULL	dry matter 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that the intercellular matrix of Bacillus subtilis 271 mainly consists of alpha-1 , 4 - glucan ( 65 % of dry matter ) , branched at some C-3 residues of the polymeric chain , and poly-D-glutamic acid ( 19 % of dry matter ) .
	manualset3
109839	6	402005	13	NULL	NULL	0	NULL	C-3 residues 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that the intercellular matrix of Bacillus subtilis 271 mainly consists of alpha-1 , 4 - glucan ( 65 % of dry matter ) , branched at some C-3 residues of the polymeric chain , and poly-D-glutamic acid ( 19 % of dry matter ) .
	manualset3
109840	7	402005	13	NULL	NULL	0	NULL	polymeric chain	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that the intercellular matrix of Bacillus subtilis 271 mainly consists of alpha-1 , 4 - glucan ( 65 % of dry matter ) , branched at some C-3 residues of the polymeric chain , and poly-D-glutamic acid ( 19 % of dry matter ) .
	manualset3
109841	8	402005	13	NULL	NULL	0	NULL	poly-D-glutamic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that the intercellular matrix of Bacillus subtilis 271 mainly consists of alpha-1 , 4 - glucan ( 65 % of dry matter ) , branched at some C-3 residues of the polymeric chain , and poly-D-glutamic acid ( 19 % of dry matter ) .
	manualset3
109842	9	402005	13	NULL	NULL	0	NULL	19 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that the intercellular matrix of Bacillus subtilis 271 mainly consists of alpha-1 , 4 - glucan ( 65 % of dry matter ) , branched at some C-3 residues of the polymeric chain , and poly-D-glutamic acid ( 19 % of dry matter ) .
	manualset3
109843	10	402005	13	NULL	NULL	0	NULL	dry matter	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that the intercellular matrix of Bacillus subtilis 271 mainly consists of alpha-1 , 4 - glucan ( 65 % of dry matter ) , branched at some C-3 residues of the polymeric chain , and poly-D-glutamic acid ( 19 % of dry matter ) .
	manualset3
109844	1	402006	13	NULL	NULL	0	NULL	change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that the most characteristic change was an increase in the latency of wave III on the affected side .
	manualset3
109845	2	402006	13	NULL	NULL	0	NULL	latency of wave III	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that the most characteristic change was an increase in the latency of wave III on the affected side .
	manualset3
109846	3	402006	13	NULL	NULL	0	NULL	affected side 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that the most characteristic change was an increase in the latency of wave III on the affected side .
	manualset3
109847	4	402006	13	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that the most characteristic change was an increase in the latency of wave III on the affected side .
	manualset3
109848	1	402007	13	NULL	NULL	0	NULL	nucleophilicities	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that the nucleophilicities of all the halides were lower in all of the ionic liquids than in dichloromethane .
	manualset3
109849	2	402007	13	NULL	NULL	0	NULL	 halides 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that the nucleophilicities of all the halides were lower in all of the ionic liquids than in dichloromethane .
	manualset3
109850	3	402007	13	NULL	NULL	0	NULL	ionic liquids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that the nucleophilicities of all the halides were lower in all of the ionic liquids than in dichloromethane .
	manualset3
109851	4	402007	13	NULL	NULL	0	NULL	dichloromethane	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that the nucleophilicities of all the halides were lower in all of the ionic liquids than in dichloromethane .
	manualset3
109852	1	402008	13	NULL	NULL	0	NULL	postoperative changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that the postoperative changes that occur in the axial inclination of the lower incisors are small enough to be clinically insignificant , provided an adequate overbite has been established .
	manualset3
109853	2	402008	13	NULL	NULL	NULL	NULL	axial inclination 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was found that the postoperative changes that occur in the axial inclination of the lower incisors are small enough to be clinically insignificant , provided an adequate overbite has been established .
	manualset3
109854	3	402008	13	NULL	NULL	0	NULL	lower incisors	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that the postoperative changes that occur in the axial inclination of the lower incisors are small enough to be clinically insignificant , provided an adequate overbite has been established .
	manualset3
109855	4	402008	13	NULL	NULL	0	NULL	adequate overbite 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that the postoperative changes that occur in the axial inclination of the lower incisors are small enough to be clinically insignificant , provided an adequate overbite has been established .
	manualset3
109856	1	402009	13	NULL	NULL	0	NULL	rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that the rate of deactivation increases abruptly on raising the temperature in the region of the gel-liquid phase transition of the lipid bilayer ( 41 degrees C ) .
	manualset3
109857	2	402009	13	NULL	NULL	0	NULL	deactivation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that the rate of deactivation increases abruptly on raising the temperature in the region of the gel-liquid phase transition of the lipid bilayer ( 41 degrees C ) .
	manualset3
109859	4	402009	13	NULL	NULL	0	NULL	 temperature	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that the rate of deactivation increases abruptly on raising the temperature in the region of the gel-liquid phase transition of the lipid bilayer ( 41 degrees C ) .
	manualset3
109860	5	402009	13	NULL	NULL	NULL	NULL	region 	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was found that the rate of deactivation increases abruptly on raising the temperature in the region of the gel-liquid phase transition of the lipid bilayer ( 41 degrees C ) .
	manualset3
109861	6	402009	13	NULL	NULL	NULL	NULL	lipid bilayer	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was found that the rate of deactivation increases abruptly on raising the temperature in the region of the gel-liquid phase transition of the lipid bilayer ( 41 degrees C ) .
	manualset3
109862	7	402009	13	NULL	NULL	0	NULL	41 degrees C 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that the rate of deactivation increases abruptly on raising the temperature in the region of the gel-liquid phase transition of the lipid bilayer ( 41 degrees C ) .
	manualset3
109863	8	402009	13	NULL	NULL	0	NULL	gel-liquid phase transition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that the rate of deactivation increases abruptly on raising the temperature in the region of the gel-liquid phase transition of the lipid bilayer ( 41 degrees C ) .
	manualset3
109864	1	402010	13	NULL	NULL	0	NULL	whole-body irradiation ( WBI )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that whole-body irradiation ( WBI ) with X-ray doses above 0.5 Gy caused a dose-dependent depression of both UD5 and DNA polymerase activity , while low dose radiation below 250 mGy could stimulate the DNA repair synthesis and the enzyme activity .
	manualset3
109865	2	402010	13	NULL	NULL	0	NULL	X-ray doses	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that whole-body irradiation ( WBI ) with X-ray doses above 0.5 Gy caused a dose-dependent depression of both UD5 and DNA polymerase activity , while low dose radiation below 250 mGy could stimulate the DNA repair synthesis and the enzyme activity .
	manualset3
109866	3	402010	13	NULL	NULL	0	NULL	0.5 Gy	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that whole-body irradiation ( WBI ) with X-ray doses above 0.5 Gy caused a dose-dependent depression of both UD5 and DNA polymerase activity , while low dose radiation below 250 mGy could stimulate the DNA repair synthesis and the enzyme activity .
	manualset3
109867	4	402010	13	NULL	NULL	0	NULL	depression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that whole-body irradiation ( WBI ) with X-ray doses above 0.5 Gy caused a dose-dependent depression of both UD5 and DNA polymerase activity , while low dose radiation below 250 mGy could stimulate the DNA repair synthesis and the enzyme activity .
	manualset3
109868	5	402010	13	NULL	NULL	0	NULL	UD5 activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that whole-body irradiation ( WBI ) with X-ray doses above 0.5 Gy caused a dose-dependent depression of both UD5 and DNA polymerase activity , while low dose radiation below 250 mGy could stimulate the DNA repair synthesis and the enzyme activity .
	manualset3
109869	6	402010	13	NULL	NULL	0	NULL	DNA polymerase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that whole-body irradiation ( WBI ) with X-ray doses above 0.5 Gy caused a dose-dependent depression of both UD5 and DNA polymerase activity , while low dose radiation below 250 mGy could stimulate the DNA repair synthesis and the enzyme activity .
	manualset3
109870	7	402010	13	NULL	NULL	0	NULL	low dose radiation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that whole-body irradiation ( WBI ) with X-ray doses above 0.5 Gy caused a dose-dependent depression of both UD5 and DNA polymerase activity , while low dose radiation below 250 mGy could stimulate the DNA repair synthesis and the enzyme activity .
	manualset3
109871	8	402010	13	NULL	NULL	0	NULL	250 mGy	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that whole-body irradiation ( WBI ) with X-ray doses above 0.5 Gy caused a dose-dependent depression of both UD5 and DNA polymerase activity , while low dose radiation below 250 mGy could stimulate the DNA repair synthesis and the enzyme activity .
	manualset3
109872	9	402010	13	NULL	NULL	0	NULL	DNA repair synthesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that whole-body irradiation ( WBI ) with X-ray doses above 0.5 Gy caused a dose-dependent depression of both UD5 and DNA polymerase activity , while low dose radiation below 250 mGy could stimulate the DNA repair synthesis and the enzyme activity .
	manualset3
109873	10	402010	13	NULL	NULL	0	NULL	enzyme activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was found that whole-body irradiation ( WBI ) with X-ray doses above 0.5 Gy caused a dose-dependent depression of both UD5 and DNA polymerase activity , while low dose radiation below 250 mGy could stimulate the DNA repair synthesis and the enzyme activity .
	manualset3
109874	1	402011	13	NULL	NULL	0	NULL	columns of kieselguhr 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It was fractionated on columns of kieselguhr coated with methylated serum albumin and the radioactivity in fractions corresponding to transfer RNA , 7s RNA , ribosomal RNA , Q ( 1 ) - RNA , Q ( 2 ) - RNA and DNA-like RNA was determined .
	manualset3
109875	2	402011	13	NULL	NULL	0	NULL	methylated serum albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It was fractionated on columns of kieselguhr coated with methylated serum albumin and the radioactivity in fractions corresponding to transfer RNA , 7s RNA , ribosomal RNA , Q ( 1 ) - RNA , Q ( 2 ) - RNA and DNA-like RNA was determined .
	manualset3
109876	3	402011	13	NULL	NULL	0	NULL	radioactivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was fractionated on columns of kieselguhr coated with methylated serum albumin and the radioactivity in fractions corresponding to transfer RNA , 7s RNA , ribosomal RNA , Q ( 1 ) - RNA , Q ( 2 ) - RNA and DNA-like RNA was determined .
	manualset3
109877	4	402011	13	NULL	NULL	0	NULL	fractions 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It was fractionated on columns of kieselguhr coated with methylated serum albumin and the radioactivity in fractions corresponding to transfer RNA , 7s RNA , ribosomal RNA , Q ( 1 ) - RNA , Q ( 2 ) - RNA and DNA-like RNA was determined .
	manualset3
109878	5	402011	13	NULL	NULL	0	NULL	transfer RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It was fractionated on columns of kieselguhr coated with methylated serum albumin and the radioactivity in fractions corresponding to transfer RNA , 7s RNA , ribosomal RNA , Q ( 1 ) - RNA , Q ( 2 ) - RNA and DNA-like RNA was determined .
	manualset3
109879	6	402011	13	NULL	NULL	0	NULL	7s RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It was fractionated on columns of kieselguhr coated with methylated serum albumin and the radioactivity in fractions corresponding to transfer RNA , 7s RNA , ribosomal RNA , Q ( 1 ) - RNA , Q ( 2 ) - RNA and DNA-like RNA was determined .
	manualset3
109880	7	402011	13	NULL	NULL	0	NULL	ribosomal RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It was fractionated on columns of kieselguhr coated with methylated serum albumin and the radioactivity in fractions corresponding to transfer RNA , 7s RNA , ribosomal RNA , Q ( 1 ) - RNA , Q ( 2 ) - RNA and DNA-like RNA was determined .
	manualset3
109881	8	402011	13	NULL	NULL	0	NULL	Q ( 1 ) - RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It was fractionated on columns of kieselguhr coated with methylated serum albumin and the radioactivity in fractions corresponding to transfer RNA , 7s RNA , ribosomal RNA , Q ( 1 ) - RNA , Q ( 2 ) - RNA and DNA-like RNA was determined .
	manualset3
109882	9	402011	13	NULL	NULL	0	NULL	Q ( 2 ) - RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It was fractionated on columns of kieselguhr coated with methylated serum albumin and the radioactivity in fractions corresponding to transfer RNA , 7s RNA , ribosomal RNA , Q ( 1 ) - RNA , Q ( 2 ) - RNA and DNA-like RNA was determined .
	manualset3
109883	10	402011	13	NULL	NULL	0	NULL	DNA-like RNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It was fractionated on columns of kieselguhr coated with methylated serum albumin and the radioactivity in fractions corresponding to transfer RNA , 7s RNA , ribosomal RNA , Q ( 1 ) - RNA , Q ( 2 ) - RNA and DNA-like RNA was determined .
	manualset3
109884	1	402012	13	NULL	NULL	0	NULL	NF-kappaB inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was further observed that NF-kappaB inhibitor but not c-Jun N-terminal kinase inhibitor ( SP600125 ) suppressed TNF-alpha expression .
	manualset3
109885	2	402012	13	NULL	NULL	0	NULL	 c-Jun N-terminal kinase inhibitor ( SP600125 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was further observed that NF-kappaB inhibitor but not c-Jun N-terminal kinase inhibitor ( SP600125 ) suppressed TNF-alpha expression .
	manualset3
109886	3	402012	13	NULL	NULL	0	NULL	TNF-alpha expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was further observed that NF-kappaB inhibitor but not c-Jun N-terminal kinase inhibitor ( SP600125 ) suppressed TNF-alpha expression .
	manualset3
109887	1	402013	13	NULL	NULL	0	NULL	cryptococcus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It was hypothesized that cryptococcus infection induced the autoimmune mechanism which resulted in the ADEM-like exacerbation .
	manualset3
109888	2	402013	13	NULL	NULL	0	NULL	infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was hypothesized that cryptococcus infection induced the autoimmune mechanism which resulted in the ADEM-like exacerbation .
	manualset3
109889	3	402013	13	NULL	NULL	0	NULL	 autoimmune mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was hypothesized that cryptococcus infection induced the autoimmune mechanism which resulted in the ADEM-like exacerbation .
	manualset3
109890	4	402013	13	NULL	NULL	0	NULL	ADEM-like exacerbation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was hypothesized that cryptococcus infection induced the autoimmune mechanism which resulted in the ADEM-like exacerbation .
	manualset3
109891	1	402014	13	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It was hypothesized that perhaps these cells had already undergone some stage , or stages , of the progression to neoplasia , and that as a consequence of these changes , one could observe differential expression of characteristics of the transformed phenotype in these cells compared to normal , or perhaps they would behave differently in vivo .
	manualset3
109892	2	402014	13	NULL	NULL	0	NULL	stage 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was hypothesized that perhaps these cells had already undergone some stage , or stages , of the progression to neoplasia , and that as a consequence of these changes , one could observe differential expression of characteristics of the transformed phenotype in these cells compared to normal , or perhaps they would behave differently in vivo .
	manualset3
109893	3	402014	13	NULL	NULL	0	NULL	stages 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was hypothesized that perhaps these cells had already undergone some stage , or stages , of the progression to neoplasia , and that as a consequence of these changes , one could observe differential expression of characteristics of the transformed phenotype in these cells compared to normal , or perhaps they would behave differently in vivo .
	manualset3
109894	4	402014	13	NULL	NULL	0	NULL	progression to neoplasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was hypothesized that perhaps these cells had already undergone some stage , or stages , of the progression to neoplasia , and that as a consequence of these changes , one could observe differential expression of characteristics of the transformed phenotype in these cells compared to normal , or perhaps they would behave differently in vivo .
	manualset3
109895	5	402014	13	NULL	NULL	0	NULL	consequence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was hypothesized that perhaps these cells had already undergone some stage , or stages , of the progression to neoplasia , and that as a consequence of these changes , one could observe differential expression of characteristics of the transformed phenotype in these cells compared to normal , or perhaps they would behave differently in vivo .
	manualset3
109896	6	402014	13	NULL	NULL	0	NULL	changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was hypothesized that perhaps these cells had already undergone some stage , or stages , of the progression to neoplasia , and that as a consequence of these changes , one could observe differential expression of characteristics of the transformed phenotype in these cells compared to normal , or perhaps they would behave differently in vivo .
	manualset3
109897	7	402014	13	NULL	NULL	0	NULL	differential expression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was hypothesized that perhaps these cells had already undergone some stage , or stages , of the progression to neoplasia , and that as a consequence of these changes , one could observe differential expression of characteristics of the transformed phenotype in these cells compared to normal , or perhaps they would behave differently in vivo .
	manualset3
109898	8	402014	13	NULL	NULL	0	NULL	characteristics 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was hypothesized that perhaps these cells had already undergone some stage , or stages , of the progression to neoplasia , and that as a consequence of these changes , one could observe differential expression of characteristics of the transformed phenotype in these cells compared to normal , or perhaps they would behave differently in vivo .
	manualset3
109899	9	402014	13	NULL	NULL	0	NULL	 phenotype 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was hypothesized that perhaps these cells had already undergone some stage , or stages , of the progression to neoplasia , and that as a consequence of these changes , one could observe differential expression of characteristics of the transformed phenotype in these cells compared to normal , or perhaps they would behave differently in vivo .
	manualset3
109900	10	402014	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It was hypothesized that perhaps these cells had already undergone some stage , or stages , of the progression to neoplasia , and that as a consequence of these changes , one could observe differential expression of characteristics of the transformed phenotype in these cells compared to normal , or perhaps they would behave differently in vivo .
	manualset3
109901	1	402015	13	NULL	NULL	0	NULL	possibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was important to consider the possibility of a intracranial hematoma , when the disturbance of consciousness was recognized after open heart surgery and/or during anticoagulant therapy .
	manualset3
109902	2	402015	13	NULL	NULL	0	NULL	intracranial hematoma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was important to consider the possibility of a intracranial hematoma , when the disturbance of consciousness was recognized after open heart surgery and/or during anticoagulant therapy .
	manualset3
109903	3	402015	13	NULL	NULL	0	NULL	disturbance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was important to consider the possibility of a intracranial hematoma , when the disturbance of consciousness was recognized after open heart surgery and/or during anticoagulant therapy .
	manualset3
109904	4	402015	13	NULL	NULL	0	NULL	consciousness 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was important to consider the possibility of a intracranial hematoma , when the disturbance of consciousness was recognized after open heart surgery and/or during anticoagulant therapy .
	manualset3
109905	5	402015	13	NULL	NULL	0	NULL	open heart surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It was important to consider the possibility of a intracranial hematoma , when the disturbance of consciousness was recognized after open heart surgery and/or during anticoagulant therapy .
	manualset3
109906	6	402015	13	NULL	NULL	0	NULL	anticoagulant therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It was important to consider the possibility of a intracranial hematoma , when the disturbance of consciousness was recognized after open heart surgery and/or during anticoagulant therapy .
	manualset3
109907	1	402016	13	NULL	NULL	0	NULL	anti-HCV 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It was notable that anti-HCV was much less prevalent among HBsAg-positive patients with HCC or LC than among HBsAg-negative ones .
	manualset3
109908	2	402016	13	NULL	NULL	0	NULL	 HBsAg-positive patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It was notable that anti-HCV was much less prevalent among HBsAg-positive patients with HCC or LC than among HBsAg-negative ones .
	manualset3
109909	3	402016	13	NULL	NULL	0	NULL	HCC	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was notable that anti-HCV was much less prevalent among HBsAg-positive patients with HCC or LC than among HBsAg-negative ones .
	manualset3
109910	4	402016	13	NULL	NULL	0	NULL	LC	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was notable that anti-HCV was much less prevalent among HBsAg-positive patients with HCC or LC than among HBsAg-negative ones .
	manualset3
109911	5	402016	13	NULL	NULL	0	NULL	HBsAg-negative ones	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It was notable that anti-HCV was much less prevalent among HBsAg-positive patients with HCC or LC than among HBsAg-negative ones .
	manualset3
109912	1	402017	13	NULL	NULL	0	NULL	PSA age index 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was noted that PSA age index is more susceptible than PSA density to diagnose prostate cancer .
	manualset3
109913	2	402017	13	NULL	NULL	0	NULL	PSA density	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was noted that PSA age index is more susceptible than PSA density to diagnose prostate cancer .
	manualset3
109914	3	402017	13	NULL	NULL	0	NULL	prostate cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It was noted that PSA age index is more susceptible than PSA density to diagnose prostate cancer .
	manualset3
109915	1	402018	13	NULL	NULL	0	NULL	biocatalyst	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was possible to use the same biocatalyst repetitively for 25 analyses with a 10 min intermediate washing of the biocatalyst required for reestablishing the starting conditions .
	manualset3
109916	2	402018	13	NULL	NULL	0	NULL	25 analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	It was possible to use the same biocatalyst repetitively for 25 analyses with a 10 min intermediate washing of the biocatalyst required for reestablishing the starting conditions .
	manualset3
109917	3	402018	13	NULL	NULL	0	NULL	10 min 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	It was possible to use the same biocatalyst repetitively for 25 analyses with a 10 min intermediate washing of the biocatalyst required for reestablishing the starting conditions .
	manualset3
109918	4	402018	13	NULL	NULL	0	NULL	washing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was possible to use the same biocatalyst repetitively for 25 analyses with a 10 min intermediate washing of the biocatalyst required for reestablishing the starting conditions .
	manualset3
109919	5	402018	13	NULL	NULL	0	NULL	biocatalyst	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was possible to use the same biocatalyst repetitively for 25 analyses with a 10 min intermediate washing of the biocatalyst required for reestablishing the starting conditions .
	manualset3
109920	6	402018	13	NULL	NULL	0	NULL	conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	It was possible to use the same biocatalyst repetitively for 25 analyses with a 10 min intermediate washing of the biocatalyst required for reestablishing the starting conditions .
	manualset3
109921	1	402019	13	NULL	NULL	0	NULL	defect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was postulated that the defect in long-chain fatty acid oxidation in this disorder is caused by an abnormality in the mitochondrial acylcarnitine transport .
	manualset3
109922	2	402019	13	NULL	NULL	0	NULL	long-chain fatty acid oxidation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was postulated that the defect in long-chain fatty acid oxidation in this disorder is caused by an abnormality in the mitochondrial acylcarnitine transport .
	manualset3
109923	3	402019	13	NULL	NULL	0	NULL	disorder	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was postulated that the defect in long-chain fatty acid oxidation in this disorder is caused by an abnormality in the mitochondrial acylcarnitine transport .
	manualset3
109924	4	402019	13	NULL	NULL	0	NULL	abnormality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was postulated that the defect in long-chain fatty acid oxidation in this disorder is caused by an abnormality in the mitochondrial acylcarnitine transport .
	manualset3
109925	5	402019	13	NULL	NULL	0	NULL	mitochondrial acylcarnitine transport	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was postulated that the defect in long-chain fatty acid oxidation in this disorder is caused by an abnormality in the mitochondrial acylcarnitine transport .
	manualset3
109926	1	402020	13	NULL	NULL	0	NULL	 ( Pt ( O , O ' - acac ) ( - acac ) ( DMS ) )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was previously demonstrated that ( Pt ( O , O ' - acac ) ( - acac ) ( DMS ) ) exerted toxic effects at high doses , whilst sub-cytotoxic concentrations induced anoikis and decreased cell migration .
	manualset3
109927	2	402020	13	NULL	NULL	0	NULL	toxic effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was previously demonstrated that ( Pt ( O , O ' - acac ) ( - acac ) ( DMS ) ) exerted toxic effects at high doses , whilst sub-cytotoxic concentrations induced anoikis and decreased cell migration .
	manualset3
109928	3	402020	13	NULL	NULL	0	NULL	high doses	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was previously demonstrated that ( Pt ( O , O ' - acac ) ( - acac ) ( DMS ) ) exerted toxic effects at high doses , whilst sub-cytotoxic concentrations induced anoikis and decreased cell migration .
	manualset3
109929	4	402020	13	NULL	NULL	0	NULL	sub-cytotoxic concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was previously demonstrated that ( Pt ( O , O ' - acac ) ( - acac ) ( DMS ) ) exerted toxic effects at high doses , whilst sub-cytotoxic concentrations induced anoikis and decreased cell migration .
	manualset3
109930	5	402020	13	NULL	NULL	NULL	NULL	anoikis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was previously demonstrated that ( Pt ( O , O ' - acac ) ( - acac ) ( DMS ) ) exerted toxic effects at high doses , whilst sub-cytotoxic concentrations induced anoikis and decreased cell migration .
	manualset3
109931	6	402020	13	NULL	NULL	0	NULL	cell migration 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was previously demonstrated that ( Pt ( O , O ' - acac ) ( - acac ) ( DMS ) ) exerted toxic effects at high doses , whilst sub-cytotoxic concentrations induced anoikis and decreased cell migration .
	manualset3
109932	1	402021	13	NULL	NULL	0	NULL	NK cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It was previously proposed that developing NK cells express Ly49 receptors sequentially and cumulatively , until self-MHC specific receptors are expressed and inhibit new receptor expression .
	manualset3
109933	2	402021	13	NULL	NULL	0	NULL	Ly49 receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It was previously proposed that developing NK cells express Ly49 receptors sequentially and cumulatively , until self-MHC specific receptors are expressed and inhibit new receptor expression .
	manualset3
109934	3	402021	13	NULL	NULL	0	NULL	self-MHC specific receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It was previously proposed that developing NK cells express Ly49 receptors sequentially and cumulatively , until self-MHC specific receptors are expressed and inhibit new receptor expression .
	manualset3
109935	4	402021	13	NULL	NULL	0	NULL	new receptor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It was previously proposed that developing NK cells express Ly49 receptors sequentially and cumulatively , until self-MHC specific receptors are expressed and inhibit new receptor expression .
	manualset3
109936	5	402021	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was previously proposed that developing NK cells express Ly49 receptors sequentially and cumulatively , until self-MHC specific receptors are expressed and inhibit new receptor expression .
	manualset3
109937	1	402022	13	NULL	NULL	0	NULL	values K ( b )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was proved by calculated values K ( b ) and f in the following order : K ( bTX-100 ) ) K ( bCTAB ) ) K ( bSDS ) and f ( TX-100 ) ) f ( CTAB ) ) f ( SDS ) .
	manualset3
109938	2	402022	13	NULL	NULL	0	NULL	values f	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was proved by calculated values K ( b ) and f in the following order : K ( bTX-100 ) ) K ( bCTAB ) ) K ( bSDS ) and f ( TX-100 ) ) f ( CTAB ) ) f ( SDS ) .
	manualset3
109939	3	402022	13	NULL	NULL	0	NULL	order 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was proved by calculated values K ( b ) and f in the following order : K ( bTX-100 ) ) K ( bCTAB ) ) K ( bSDS ) and f ( TX-100 ) ) f ( CTAB ) ) f ( SDS ) .
	manualset3
109940	4	402022	13	NULL	NULL	NULL	NULL	K ( bTX-100 ) )	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was proved by calculated values K ( b ) and f in the following order : K ( bTX-100 ) ) K ( bCTAB ) ) K ( bSDS ) and f ( TX-100 ) ) f ( CTAB ) ) f ( SDS ) .
	manualset3
109941	5	402022	13	NULL	NULL	NULL	NULL	K ( bCTAB ) )	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was proved by calculated values K ( b ) and f in the following order : K ( bTX-100 ) ) K ( bCTAB ) ) K ( bSDS ) and f ( TX-100 ) ) f ( CTAB ) ) f ( SDS ) .
	manualset3
109942	6	402022	13	NULL	NULL	NULL	NULL	K ( bSDS ) 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was proved by calculated values K ( b ) and f in the following order : K ( bTX-100 ) ) K ( bCTAB ) ) K ( bSDS ) and f ( TX-100 ) ) f ( CTAB ) ) f ( SDS ) .
	manualset3
109943	7	402022	13	NULL	NULL	NULL	NULL	 f ( TX-100 ) )	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was proved by calculated values K ( b ) and f in the following order : K ( bTX-100 ) ) K ( bCTAB ) ) K ( bSDS ) and f ( TX-100 ) ) f ( CTAB ) ) f ( SDS ) .
	manualset3
109944	8	402022	13	NULL	NULL	NULL	NULL	f ( CTAB ) )	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was proved by calculated values K ( b ) and f in the following order : K ( bTX-100 ) ) K ( bCTAB ) ) K ( bSDS ) and f ( TX-100 ) ) f ( CTAB ) ) f ( SDS ) .
	manualset3
109945	9	402022	13	NULL	NULL	NULL	NULL	f ( SDS ) 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was proved by calculated values K ( b ) and f in the following order : K ( bTX-100 ) ) K ( bCTAB ) ) K ( bSDS ) and f ( TX-100 ) ) f ( CTAB ) ) f ( SDS ) .
	manualset3
109946	1	402023	13	NULL	NULL	0	NULL	ROS production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that ROS production is regulated differently by the rate of oxygen consumption and membrane potential , dependent on steady-state or non-equilibrium conditions .
	manualset3
109947	2	402023	13	NULL	NULL	0	NULL	rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that ROS production is regulated differently by the rate of oxygen consumption and membrane potential , dependent on steady-state or non-equilibrium conditions .
	manualset3
109948	3	402023	13	NULL	NULL	0	NULL	oxygen consumption	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that ROS production is regulated differently by the rate of oxygen consumption and membrane potential , dependent on steady-state or non-equilibrium conditions .
	manualset3
109949	4	402023	13	NULL	NULL	0	NULL	membrane potential 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that ROS production is regulated differently by the rate of oxygen consumption and membrane potential , dependent on steady-state or non-equilibrium conditions .
	manualset3
109950	5	402023	13	NULL	NULL	0	NULL	conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that ROS production is regulated differently by the rate of oxygen consumption and membrane potential , dependent on steady-state or non-equilibrium conditions .
	manualset3
109951	1	402024	13	NULL	NULL	0	NULL	global ischemia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that global ischemia induces potassium deficiency ( 94 + / - 2 mM ) in the myocyte and an increase in the level of sodium ( 72 + / - 4 mM ) and chlorine ( 42 + / - 1 mM ) in the cytoplasm compared with intact cell ( 122 + / - 2 ; 36 + / - 1 ; 24 + / - 1 mM ) .
	manualset3
109952	2	402024	13	NULL	NULL	0	NULL	potassium deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that global ischemia induces potassium deficiency ( 94 + / - 2 mM ) in the myocyte and an increase in the level of sodium ( 72 + / - 4 mM ) and chlorine ( 42 + / - 1 mM ) in the cytoplasm compared with intact cell ( 122 + / - 2 ; 36 + / - 1 ; 24 + / - 1 mM ) .
	manualset3
109953	3	402024	13	NULL	NULL	0	NULL	94 + / - 2 mM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that global ischemia induces potassium deficiency ( 94 + / - 2 mM ) in the myocyte and an increase in the level of sodium ( 72 + / - 4 mM ) and chlorine ( 42 + / - 1 mM ) in the cytoplasm compared with intact cell ( 122 + / - 2 ; 36 + / - 1 ; 24 + / - 1 mM ) .
	manualset3
109954	4	402024	13	NULL	NULL	0	NULL	myocyte	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that global ischemia induces potassium deficiency ( 94 + / - 2 mM ) in the myocyte and an increase in the level of sodium ( 72 + / - 4 mM ) and chlorine ( 42 + / - 1 mM ) in the cytoplasm compared with intact cell ( 122 + / - 2 ; 36 + / - 1 ; 24 + / - 1 mM ) .
	manualset3
109955	5	402024	13	NULL	NULL	0	NULL	level of sodium	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that global ischemia induces potassium deficiency ( 94 + / - 2 mM ) in the myocyte and an increase in the level of sodium ( 72 + / - 4 mM ) and chlorine ( 42 + / - 1 mM ) in the cytoplasm compared with intact cell ( 122 + / - 2 ; 36 + / - 1 ; 24 + / - 1 mM ) .
	manualset3
109956	6	402024	13	NULL	NULL	0	NULL	72 + / - 4 mM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that global ischemia induces potassium deficiency ( 94 + / - 2 mM ) in the myocyte and an increase in the level of sodium ( 72 + / - 4 mM ) and chlorine ( 42 + / - 1 mM ) in the cytoplasm compared with intact cell ( 122 + / - 2 ; 36 + / - 1 ; 24 + / - 1 mM ) .
	manualset3
109957	7	402024	13	NULL	NULL	0	NULL	chlorine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that global ischemia induces potassium deficiency ( 94 + / - 2 mM ) in the myocyte and an increase in the level of sodium ( 72 + / - 4 mM ) and chlorine ( 42 + / - 1 mM ) in the cytoplasm compared with intact cell ( 122 + / - 2 ; 36 + / - 1 ; 24 + / - 1 mM ) .
	manualset3
109958	8	402024	13	NULL	NULL	0	NULL	42 + / - 1 mM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that global ischemia induces potassium deficiency ( 94 + / - 2 mM ) in the myocyte and an increase in the level of sodium ( 72 + / - 4 mM ) and chlorine ( 42 + / - 1 mM ) in the cytoplasm compared with intact cell ( 122 + / - 2 ; 36 + / - 1 ; 24 + / - 1 mM ) .
	manualset3
109959	9	402024	13	NULL	NULL	0	NULL	cytoplasm	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that global ischemia induces potassium deficiency ( 94 + / - 2 mM ) in the myocyte and an increase in the level of sodium ( 72 + / - 4 mM ) and chlorine ( 42 + / - 1 mM ) in the cytoplasm compared with intact cell ( 122 + / - 2 ; 36 + / - 1 ; 24 + / - 1 mM ) .
	manualset3
109960	10	402024	13	NULL	NULL	0	NULL	intact cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that global ischemia induces potassium deficiency ( 94 + / - 2 mM ) in the myocyte and an increase in the level of sodium ( 72 + / - 4 mM ) and chlorine ( 42 + / - 1 mM ) in the cytoplasm compared with intact cell ( 122 + / - 2 ; 36 + / - 1 ; 24 + / - 1 mM ) .
	manualset3
109961	11	402024	13	NULL	NULL	0	NULL	122 + / - 2 ; 36 + / - 1 ; 24 + / - 1 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that global ischemia induces potassium deficiency ( 94 + / - 2 mM ) in the myocyte and an increase in the level of sodium ( 72 + / - 4 mM ) and chlorine ( 42 + / - 1 mM ) in the cytoplasm compared with intact cell ( 122 + / - 2 ; 36 + / - 1 ; 24 + / - 1 mM ) .
	manualset3
109962	1	402025	13	NULL	NULL	0	NULL	surface proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that surface proteins were involved in the adhesion of L15 to flounder mucus .
	manualset3
109963	2	402025	13	NULL	NULL	0	NULL	adhesion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that surface proteins were involved in the adhesion of L15 to flounder mucus .
	manualset3
109964	3	402025	13	NULL	NULL	0	NULL	 L15	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that surface proteins were involved in the adhesion of L15 to flounder mucus .
	manualset3
109965	4	402025	13	NULL	NULL	0	NULL	flounder mucus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that surface proteins were involved in the adhesion of L15 to flounder mucus .
	manualset3
109966	1	402026	13	NULL	NULL	0	NULL	conversion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that the conversion of PC was nearly 100 % , and the yield of bisphenol A ( BPA ) was over 95 % under the following conditions : m ( ( Bmim ) ( Ac ) ) : m ( PC ) = 0.75 : 1 ; m ( methanol ) : m ( PC ) = 0.75 : 1 ; a reaction temperature of 90 C and a total time of 2.5 h. The ionic liquid could be reused up to 6 times with no apparent decrease in the conversion of PC and yield of BPA .
	manualset3
109967	2	402026	13	NULL	NULL	0	NULL	PC 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that the conversion of PC was nearly 100 % , and the yield of bisphenol A ( BPA ) was over 95 % under the following conditions : m ( ( Bmim ) ( Ac ) ) : m ( PC ) = 0.75 : 1 ; m ( methanol ) : m ( PC ) = 0.75 : 1 ; a reaction temperature of 90 C and a total time of 2.5 h. The ionic liquid could be reused up to 6 times with no apparent decrease in the conversion of PC and yield of BPA .
	manualset3
109968	3	402026	13	NULL	NULL	0	NULL	100 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that the conversion of PC was nearly 100 % , and the yield of bisphenol A ( BPA ) was over 95 % under the following conditions : m ( ( Bmim ) ( Ac ) ) : m ( PC ) = 0.75 : 1 ; m ( methanol ) : m ( PC ) = 0.75 : 1 ; a reaction temperature of 90 C and a total time of 2.5 h. The ionic liquid could be reused up to 6 times with no apparent decrease in the conversion of PC and yield of BPA .
	manualset3
109969	4	402026	13	NULL	NULL	0	NULL	 yield	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that the conversion of PC was nearly 100 % , and the yield of bisphenol A ( BPA ) was over 95 % under the following conditions : m ( ( Bmim ) ( Ac ) ) : m ( PC ) = 0.75 : 1 ; m ( methanol ) : m ( PC ) = 0.75 : 1 ; a reaction temperature of 90 C and a total time of 2.5 h. The ionic liquid could be reused up to 6 times with no apparent decrease in the conversion of PC and yield of BPA .
	manualset3
109970	5	402026	13	NULL	NULL	0	NULL	bisphenol A ( BPA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that the conversion of PC was nearly 100 % , and the yield of bisphenol A ( BPA ) was over 95 % under the following conditions : m ( ( Bmim ) ( Ac ) ) : m ( PC ) = 0.75 : 1 ; m ( methanol ) : m ( PC ) = 0.75 : 1 ; a reaction temperature of 90 C and a total time of 2.5 h. The ionic liquid could be reused up to 6 times with no apparent decrease in the conversion of PC and yield of BPA .
	manualset3
109971	6	402026	13	NULL	NULL	0	NULL	95 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that the conversion of PC was nearly 100 % , and the yield of bisphenol A ( BPA ) was over 95 % under the following conditions : m ( ( Bmim ) ( Ac ) ) : m ( PC ) = 0.75 : 1 ; m ( methanol ) : m ( PC ) = 0.75 : 1 ; a reaction temperature of 90 C and a total time of 2.5 h. The ionic liquid could be reused up to 6 times with no apparent decrease in the conversion of PC and yield of BPA .
	manualset3
109972	7	402026	13	NULL	NULL	0	NULL	conditions 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that the conversion of PC was nearly 100 % , and the yield of bisphenol A ( BPA ) was over 95 % under the following conditions : m ( ( Bmim ) ( Ac ) ) : m ( PC ) = 0.75 : 1 ; m ( methanol ) : m ( PC ) = 0.75 : 1 ; a reaction temperature of 90 C and a total time of 2.5 h. The ionic liquid could be reused up to 6 times with no apparent decrease in the conversion of PC and yield of BPA .
	manualset3
109973	8	402026	13	NULL	NULL	0	NULL	m ( ( Bmim ) ( Ac ) ) : m ( PC ) = 0.75 : 1 ; m ( methanol ) : m ( PC ) = 0.75 : 1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that the conversion of PC was nearly 100 % , and the yield of bisphenol A ( BPA ) was over 95 % under the following conditions : m ( ( Bmim ) ( Ac ) ) : m ( PC ) = 0.75 : 1 ; m ( methanol ) : m ( PC ) = 0.75 : 1 ; a reaction temperature of 90 C and a total time of 2.5 h. The ionic liquid could be reused up to 6 times with no apparent decrease in the conversion of PC and yield of BPA .
	manualset3
109974	9	402026	13	NULL	NULL	0	NULL	reaction temperature	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that the conversion of PC was nearly 100 % , and the yield of bisphenol A ( BPA ) was over 95 % under the following conditions : m ( ( Bmim ) ( Ac ) ) : m ( PC ) = 0.75 : 1 ; m ( methanol ) : m ( PC ) = 0.75 : 1 ; a reaction temperature of 90 C and a total time of 2.5 h. The ionic liquid could be reused up to 6 times with no apparent decrease in the conversion of PC and yield of BPA .
	manualset3
109975	10	402026	13	NULL	NULL	0	NULL	90 C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that the conversion of PC was nearly 100 % , and the yield of bisphenol A ( BPA ) was over 95 % under the following conditions : m ( ( Bmim ) ( Ac ) ) : m ( PC ) = 0.75 : 1 ; m ( methanol ) : m ( PC ) = 0.75 : 1 ; a reaction temperature of 90 C and a total time of 2.5 h. The ionic liquid could be reused up to 6 times with no apparent decrease in the conversion of PC and yield of BPA .
	manualset3
109976	11	402026	13	NULL	NULL	0	NULL	total time of 2.5 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that the conversion of PC was nearly 100 % , and the yield of bisphenol A ( BPA ) was over 95 % under the following conditions : m ( ( Bmim ) ( Ac ) ) : m ( PC ) = 0.75 : 1 ; m ( methanol ) : m ( PC ) = 0.75 : 1 ; a reaction temperature of 90 C and a total time of 2.5 h. The ionic liquid could be reused up to 6 times with no apparent decrease in the conversion of PC and yield of BPA .
	manualset3
109977	12	402026	13	NULL	NULL	0	NULL	ionic liquid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that the conversion of PC was nearly 100 % , and the yield of bisphenol A ( BPA ) was over 95 % under the following conditions : m ( ( Bmim ) ( Ac ) ) : m ( PC ) = 0.75 : 1 ; m ( methanol ) : m ( PC ) = 0.75 : 1 ; a reaction temperature of 90 C and a total time of 2.5 h. The ionic liquid could be reused up to 6 times with no apparent decrease in the conversion of PC and yield of BPA .
	manualset3
109978	13	402026	13	NULL	NULL	0	NULL	6 times	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that the conversion of PC was nearly 100 % , and the yield of bisphenol A ( BPA ) was over 95 % under the following conditions : m ( ( Bmim ) ( Ac ) ) : m ( PC ) = 0.75 : 1 ; m ( methanol ) : m ( PC ) = 0.75 : 1 ; a reaction temperature of 90 C and a total time of 2.5 h. The ionic liquid could be reused up to 6 times with no apparent decrease in the conversion of PC and yield of BPA .
	manualset3
109979	14	402026	13	NULL	NULL	0	NULL	conversion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that the conversion of PC was nearly 100 % , and the yield of bisphenol A ( BPA ) was over 95 % under the following conditions : m ( ( Bmim ) ( Ac ) ) : m ( PC ) = 0.75 : 1 ; m ( methanol ) : m ( PC ) = 0.75 : 1 ; a reaction temperature of 90 C and a total time of 2.5 h. The ionic liquid could be reused up to 6 times with no apparent decrease in the conversion of PC and yield of BPA .
	manualset3
109980	15	402026	13	NULL	NULL	0	NULL	PC	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that the conversion of PC was nearly 100 % , and the yield of bisphenol A ( BPA ) was over 95 % under the following conditions : m ( ( Bmim ) ( Ac ) ) : m ( PC ) = 0.75 : 1 ; m ( methanol ) : m ( PC ) = 0.75 : 1 ; a reaction temperature of 90 C and a total time of 2.5 h. The ionic liquid could be reused up to 6 times with no apparent decrease in the conversion of PC and yield of BPA .
	manualset3
109981	16	402026	13	NULL	NULL	0	NULL	yield	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that the conversion of PC was nearly 100 % , and the yield of bisphenol A ( BPA ) was over 95 % under the following conditions : m ( ( Bmim ) ( Ac ) ) : m ( PC ) = 0.75 : 1 ; m ( methanol ) : m ( PC ) = 0.75 : 1 ; a reaction temperature of 90 C and a total time of 2.5 h. The ionic liquid could be reused up to 6 times with no apparent decrease in the conversion of PC and yield of BPA .
	manualset3
109982	17	402026	13	NULL	NULL	0	NULL	BPA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that the conversion of PC was nearly 100 % , and the yield of bisphenol A ( BPA ) was over 95 % under the following conditions : m ( ( Bmim ) ( Ac ) ) : m ( PC ) = 0.75 : 1 ; m ( methanol ) : m ( PC ) = 0.75 : 1 ; a reaction temperature of 90 C and a total time of 2.5 h. The ionic liquid could be reused up to 6 times with no apparent decrease in the conversion of PC and yield of BPA .
	manualset3
109983	1	402027	13	NULL	NULL	0	NULL	entrapped molecules 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that the entrapped molecules can be released from the capsules by controlling the hydration of the polymer , which in turn changes the permeability of the oil content through the polypyrrole shells .
	manualset3
109984	2	402027	13	NULL	NULL	0	NULL	capsules 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that the entrapped molecules can be released from the capsules by controlling the hydration of the polymer , which in turn changes the permeability of the oil content through the polypyrrole shells .
	manualset3
109985	3	402027	13	NULL	NULL	0	NULL	hydration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that the entrapped molecules can be released from the capsules by controlling the hydration of the polymer , which in turn changes the permeability of the oil content through the polypyrrole shells .
	manualset3
109986	4	402027	13	NULL	NULL	0	NULL	polymer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that the entrapped molecules can be released from the capsules by controlling the hydration of the polymer , which in turn changes the permeability of the oil content through the polypyrrole shells .
	manualset3
109987	5	402027	13	NULL	NULL	0	NULL	permeability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that the entrapped molecules can be released from the capsules by controlling the hydration of the polymer , which in turn changes the permeability of the oil content through the polypyrrole shells .
	manualset3
109988	6	402027	13	NULL	NULL	0	NULL	oil content	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that the entrapped molecules can be released from the capsules by controlling the hydration of the polymer , which in turn changes the permeability of the oil content through the polypyrrole shells .
	manualset3
109989	7	402027	13	NULL	NULL	0	NULL	polypyrrole shells	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that the entrapped molecules can be released from the capsules by controlling the hydration of the polymer , which in turn changes the permeability of the oil content through the polypyrrole shells .
	manualset3
109990	1	402028	13	NULL	NULL	0	NULL	tryptophan	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that tryptophan located inside of peptide can be exhibited on a surface and accessible to antibody .
	manualset3
109991	2	402028	13	NULL	NULL	0	NULL	peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that tryptophan located inside of peptide can be exhibited on a surface and accessible to antibody .
	manualset3
109992	3	402028	13	NULL	NULL	0	NULL	surface	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that tryptophan located inside of peptide can be exhibited on a surface and accessible to antibody .
	manualset3
109993	4	402028	13	NULL	NULL	0	NULL	antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that tryptophan located inside of peptide can be exhibited on a surface and accessible to antibody .
	manualset3
109994	1	402029	13	NULL	NULL	0	NULL	experimental conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	It was studied under various experimental conditions which allow the recognition of calcium antagonistic activity .
	manualset3
109995	2	402029	13	NULL	NULL	0	NULL	recognition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was studied under various experimental conditions which allow the recognition of calcium antagonistic activity .
	manualset3
109996	3	402029	13	NULL	NULL	0	NULL	calcium antagonistic activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was studied under various experimental conditions which allow the recognition of calcium antagonistic activity .
	manualset3
109997	1	402030	13	NULL	NULL	0	NULL	purpose	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was the purpose of the study to test the efficacy of dissolvent tablets containing mutanase and protease in preventing formation of plaque on the fitting surface of complete dentures .
	manualset3
109999	3	402030	13	NULL	NULL	0	NULL	efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It was the purpose of the study to test the efficacy of dissolvent tablets containing mutanase and protease in preventing formation of plaque on the fitting surface of complete dentures .
	manualset3
110000	4	402030	13	NULL	NULL	0	NULL	dissolvent tablets	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	It was the purpose of the study to test the efficacy of dissolvent tablets containing mutanase and protease in preventing formation of plaque on the fitting surface of complete dentures .
	manualset3
110001	5	402030	13	NULL	NULL	0	NULL	mutanase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It was the purpose of the study to test the efficacy of dissolvent tablets containing mutanase and protease in preventing formation of plaque on the fitting surface of complete dentures .
	manualset3
110002	6	402030	13	NULL	NULL	0	NULL	protease 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It was the purpose of the study to test the efficacy of dissolvent tablets containing mutanase and protease in preventing formation of plaque on the fitting surface of complete dentures .
	manualset3
110003	7	402030	13	NULL	NULL	0	NULL	formation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was the purpose of the study to test the efficacy of dissolvent tablets containing mutanase and protease in preventing formation of plaque on the fitting surface of complete dentures .
	manualset3
110004	8	402030	13	NULL	NULL	0	NULL	plaque	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was the purpose of the study to test the efficacy of dissolvent tablets containing mutanase and protease in preventing formation of plaque on the fitting surface of complete dentures .
	manualset3
110005	9	402030	13	NULL	NULL	NULL	NULL	fitting surface	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was the purpose of the study to test the efficacy of dissolvent tablets containing mutanase and protease in preventing formation of plaque on the fitting surface of complete dentures .
	manualset3
110006	10	402030	13	NULL	NULL	0	NULL	complete dentures	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	It was the purpose of the study to test the efficacy of dissolvent tablets containing mutanase and protease in preventing formation of plaque on the fitting surface of complete dentures .
	manualset3
112688	1	402231	13	NULL	NULL	0	NULL	Lead	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Lead and cadmium in soils and vegetables from urban gardens of Salamanca ( Spain ) .
	manualset3
112689	2	402231	13	NULL	NULL	0	NULL	cadmium 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Lead and cadmium in soils and vegetables from urban gardens of Salamanca ( Spain ) .
	manualset3
112690	3	402231	13	NULL	NULL	0	NULL	soils	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Lead and cadmium in soils and vegetables from urban gardens of Salamanca ( Spain ) .
	manualset3
112691	4	402231	13	NULL	NULL	0	NULL	vegetables	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Lead and cadmium in soils and vegetables from urban gardens of Salamanca ( Spain ) .
	manualset3
112692	5	402231	13	NULL	NULL	0	NULL	urban gardens	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Lead and cadmium in soils and vegetables from urban gardens of Salamanca ( Spain ) .
	manualset3
112693	6	402231	13	NULL	NULL	0	NULL	Salamanca ( Spain )	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Lead and cadmium in soils and vegetables from urban gardens of Salamanca ( Spain ) .
	manualset3
112694	1	402232	13	NULL	NULL	0	NULL	Leadership	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Leadership and the ACR : a road map to success .
	manualset3
112695	2	402232	13	NULL	NULL	0	NULL	ACR	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Leadership and the ACR : a road map to success .
	manualset3
112696	3	402232	13	NULL	NULL	0	NULL	 road map	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Leadership and the ACR : a road map to success .
	manualset3
112697	4	402232	13	NULL	NULL	0	NULL	success	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Leadership and the ACR : a road map to success .
	manualset3
112698	1	402233	13	NULL	NULL	0	NULL	Leaf 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Leaf H2O2 content increased even though total CAT activity doubled under severe drought conditions .
	manualset3
112699	2	402233	13	NULL	NULL	0	NULL	H2O2 content	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Leaf H2O2 content increased even though total CAT activity doubled under severe drought conditions .
	manualset3
112700	3	402233	13	NULL	NULL	0	NULL	total	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Leaf H2O2 content increased even though total CAT activity doubled under severe drought conditions .
	manualset3
112701	4	402233	13	NULL	NULL	0	NULL	CAT activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Leaf H2O2 content increased even though total CAT activity doubled under severe drought conditions .
	manualset3
112702	5	402233	13	NULL	NULL	0	NULL	drought conditions 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Leaf H2O2 content increased even though total CAT activity doubled under severe drought conditions .
	manualset3
112703	1	402234	13	NULL	NULL	0	NULL	Learning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Learning by honeybees ( Apis mellifera ) on arrival at and departure from a feeding place .
	manualset3
112704	2	402234	13	NULL	NULL	0	NULL	honeybees ( Apis mellifera ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Learning by honeybees ( Apis mellifera ) on arrival at and departure from a feeding place .
	manualset3
112705	3	402234	13	NULL	NULL	0	NULL	arrival	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Learning by honeybees ( Apis mellifera ) on arrival at and departure from a feeding place .
	manualset3
112706	4	402234	13	NULL	NULL	0	NULL	departure 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Learning by honeybees ( Apis mellifera ) on arrival at and departure from a feeding place .
	manualset3
112707	5	402234	13	NULL	NULL	0	NULL	feeding place	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Learning by honeybees ( Apis mellifera ) on arrival at and departure from a feeding place .
	manualset3
112708	1	402235	13	NULL	NULL	0	NULL	lessons	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Learning the lessons from the UK and other large system deployments might enable other countries to leap to the forefront of health care computing .
	manualset3
112709	2	402235	13	NULL	NULL	0	NULL	UK	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Learning the lessons from the UK and other large system deployments might enable other countries to leap to the forefront of health care computing .
	manualset3
112710	3	402235	13	NULL	NULL	0	NULL	large system deployments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Learning the lessons from the UK and other large system deployments might enable other countries to leap to the forefront of health care computing .
	manualset3
112711	4	402235	13	NULL	NULL	0	NULL	countries	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Learning the lessons from the UK and other large system deployments might enable other countries to leap to the forefront of health care computing .
	manualset3
112712	5	402235	13	NULL	NULL	0	NULL	forefront	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Learning the lessons from the UK and other large system deployments might enable other countries to leap to the forefront of health care computing .
	manualset3
112713	6	402235	13	NULL	NULL	NULL	NULL	health care computing	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Learning the lessons from the UK and other large system deployments might enable other countries to leap to the forefront of health care computing .
	manualset3
112714	1	402236	13	NULL	NULL	NULL	NULL	Learning 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Learning to fear suffocation : a new paradigm for interoceptive fear conditioning .
	manualset3
112715	2	402236	13	NULL	NULL	0	NULL	suffocation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Learning to fear suffocation : a new paradigm for interoceptive fear conditioning .
	manualset3
112716	3	402236	13	NULL	NULL	0	NULL	paradigm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Learning to fear suffocation : a new paradigm for interoceptive fear conditioning .
	manualset3
112717	4	402236	13	NULL	NULL	NULL	NULL	interoceptive fear 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Learning to fear suffocation : a new paradigm for interoceptive fear conditioning .
	manualset3
112718	5	402236	13	NULL	NULL	NULL	NULL	conditioning 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Learning to fear suffocation : a new paradigm for interoceptive fear conditioning .
	manualset3
112719	1	402237	13	NULL	NULL	NULL	NULL	Learning	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Learning to predict human error : issues of acceptability , reliability and validity .
	manualset3
112720	2	402237	13	NULL	NULL	0	NULL	human error 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Learning to predict human error : issues of acceptability , reliability and validity .
	manualset3
112721	3	402237	13	NULL	NULL	0	NULL	acceptability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Learning to predict human error : issues of acceptability , reliability and validity .
	manualset3
112722	4	402237	13	NULL	NULL	0	NULL	reliability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Learning to predict human error : issues of acceptability , reliability and validity .
	manualset3
112723	5	402237	13	NULL	NULL	0	NULL	validity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Learning to predict human error : issues of acceptability , reliability and validity .
	manualset3
112724	1	402238	13	NULL	NULL	NULL	NULL	Leber hereditary optic neuropathy	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Leber hereditary optic neuropathy associated with malabsorption syndrome after bariatric surgery .
	manualset3
112725	2	402238	13	NULL	NULL	0	NULL	malabsorption syndrome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Leber hereditary optic neuropathy associated with malabsorption syndrome after bariatric surgery .
	manualset3
112726	3	402238	13	NULL	NULL	0	NULL	bariatric surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Leber hereditary optic neuropathy associated with malabsorption syndrome after bariatric surgery .
	manualset3
112727	1	402239	13	NULL	NULL	0	NULL	Lectin I ( II ) determinants	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lectin I ( II ) determinants ( i.e. Gal beta 1 -- 3 ( 4 ) GlcNAc residues ) can be found at the nonreducing end of the carbohydrate chains derived from either N-glycosidic or O-glycosidic linkages .
	manualset3
112728	2	402239	13	NULL	NULL	0	NULL	Gal beta 1 -- 3 ( 4 ) GlcNAc residues	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lectin I ( II ) determinants ( i.e. Gal beta 1 -- 3 ( 4 ) GlcNAc residues ) can be found at the nonreducing end of the carbohydrate chains derived from either N-glycosidic or O-glycosidic linkages .
	manualset3
112729	3	402239	13	NULL	NULL	0	NULL	carbohydrate chains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lectin I ( II ) determinants ( i.e. Gal beta 1 -- 3 ( 4 ) GlcNAc residues ) can be found at the nonreducing end of the carbohydrate chains derived from either N-glycosidic or O-glycosidic linkages .
	manualset3
112730	4	402239	13	NULL	NULL	0	NULL	N-glycosidic linkages	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lectin I ( II ) determinants ( i.e. Gal beta 1 -- 3 ( 4 ) GlcNAc residues ) can be found at the nonreducing end of the carbohydrate chains derived from either N-glycosidic or O-glycosidic linkages .
	manualset3
112731	5	402239	13	NULL	NULL	0	NULL	O-glycosidic linkages	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lectin I ( II ) determinants ( i.e. Gal beta 1 -- 3 ( 4 ) GlcNAc residues ) can be found at the nonreducing end of the carbohydrate chains derived from either N-glycosidic or O-glycosidic linkages .
	manualset3
112732	1	402240	13	NULL	NULL	0	NULL	3.2-kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A 3.2-kg newborn was intubated for neonatal respiratory distress owing to a congenital tracheal stenosis .
	manualset3
112733	2	402240	13	NULL	NULL	0	NULL	newborn 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A 3.2-kg newborn was intubated for neonatal respiratory distress owing to a congenital tracheal stenosis .
	manualset3
112734	3	402240	13	NULL	NULL	0	NULL	neonatal respiratory distress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 3.2-kg newborn was intubated for neonatal respiratory distress owing to a congenital tracheal stenosis .
	manualset3
112735	4	402240	13	NULL	NULL	0	NULL	congenital tracheal stenosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 3.2-kg newborn was intubated for neonatal respiratory distress owing to a congenital tracheal stenosis .
	manualset3
112809	1	402241	13	NULL	NULL	0	NULL	Leersia hexandra Swartz ( Gramineae )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Leersia hexandra Swartz ( Gramineae ) , which occurs in Southern China , has been found to be a new chromium hyperaccumulator by means of field survey and pot-culture experiment .
	manualset3
112810	2	402241	13	NULL	NULL	0	NULL	Southern China	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Leersia hexandra Swartz ( Gramineae ) , which occurs in Southern China , has been found to be a new chromium hyperaccumulator by means of field survey and pot-culture experiment .
	manualset3
112811	3	402241	13	NULL	NULL	0	NULL	new chromium hyperaccumulator	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Leersia hexandra Swartz ( Gramineae ) , which occurs in Southern China , has been found to be a new chromium hyperaccumulator by means of field survey and pot-culture experiment .
	manualset3
112812	4	402241	13	NULL	NULL	0	NULL	field survey	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Leersia hexandra Swartz ( Gramineae ) , which occurs in Southern China , has been found to be a new chromium hyperaccumulator by means of field survey and pot-culture experiment .
	manualset3
112813	5	402241	13	NULL	NULL	0	NULL	pot-culture experiment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Leersia hexandra Swartz ( Gramineae ) , which occurs in Southern China , has been found to be a new chromium hyperaccumulator by means of field survey and pot-culture experiment .
	manualset3
112814	1	402242	13	NULL	NULL	0	NULL	Left atrial hypertrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Left atrial hypertrophy was discovered primarily by echo-CG and MCG .
	manualset3
112815	2	402242	13	NULL	NULL	0	NULL	echo-CG	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Left atrial hypertrophy was discovered primarily by echo-CG and MCG .
	manualset3
112816	3	402242	13	NULL	NULL	0	NULL	MCG	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Left atrial hypertrophy was discovered primarily by echo-CG and MCG .
	manualset3
112817	1	402243	13	NULL	NULL	0	NULL	Left hepatectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Left hepatectomy and excision of the duplication were curative .
	manualset3
112818	2	402243	13	NULL	NULL	0	NULL	excision	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Left hepatectomy and excision of the duplication were curative .
	manualset3
112819	3	402243	13	NULL	NULL	0	NULL	duplication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Left hepatectomy and excision of the duplication were curative .
	manualset3
112820	1	402244	13	NULL	NULL	0	NULL	Left ventricular ( LV ) dP/dt	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Left ventricular ( LV ) dP/dt was higher in W than in M ( p less than .005 ) .
	manualset3
112822	2	402244	13	NULL	NULL	0	NULL	W	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Left ventricular ( LV ) dP/dt was higher in W than in M ( p less than .005 ) .
	manualset3
112823	3	402244	13	NULL	NULL	0	NULL	M	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Left ventricular ( LV ) dP/dt was higher in W than in M ( p less than .005 ) .
	manualset3
112824	4	402244	13	NULL	NULL	0	NULL	p less than .005 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Left ventricular ( LV ) dP/dt was higher in W than in M ( p less than .005 ) .
	manualset3
112825	1	402245	13	NULL	NULL	0	NULL	Left ventricular dilatation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Left ventricular dilatation and elasticity of the left ventricular wall -- ultrasound cardiographic evaluation ) .
	manualset3
112826	2	402245	13	NULL	NULL	0	NULL	Left ventricular elasticity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Left ventricular dilatation and elasticity of the left ventricular wall -- ultrasound cardiographic evaluation ) .
	manualset3
112827	3	402245	13	NULL	NULL	0	NULL	left ventricular wall	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Left ventricular dilatation and elasticity of the left ventricular wall -- ultrasound cardiographic evaluation ) .
	manualset3
112828	4	402245	13	NULL	NULL	0	NULL	ultrasound cardiographic evaluation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Left ventricular dilatation and elasticity of the left ventricular wall -- ultrasound cardiographic evaluation ) .
	manualset3
112829	1	402246	13	NULL	NULL	0	NULL	Left ventricular pressure-volume ( P-V ) loops	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Left ventricular pressure-volume ( P-V ) loops provide a complete definition of cardiac performance but have been difficult to obtain in the clinical setting .
	manualset3
112830	2	402246	13	NULL	NULL	0	NULL	complete definition 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Left ventricular pressure-volume ( P-V ) loops provide a complete definition of cardiac performance but have been difficult to obtain in the clinical setting .
	manualset3
112831	3	402246	13	NULL	NULL	0	NULL	cardiac performance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Left ventricular pressure-volume ( P-V ) loops provide a complete definition of cardiac performance but have been difficult to obtain in the clinical setting .
	manualset3
112832	4	402246	13	NULL	NULL	0	NULL	clinical setting 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Left ventricular pressure-volume ( P-V ) loops provide a complete definition of cardiac performance but have been difficult to obtain in the clinical setting .
	manualset3
112833	1	402247	13	NULL	NULL	0	NULL	3 Megabase deletion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A 3 Megabase deletion in the Xq25 region , encompassing the SH2D1A gene , was defined by SNP array genotyping .
	manualset3
112834	2	402247	13	NULL	NULL	0	NULL	Xq25 region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A 3 Megabase deletion in the Xq25 region , encompassing the SH2D1A gene , was defined by SNP array genotyping .
	manualset3
112835	3	402247	13	NULL	NULL	0	NULL	SH2D1A gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A 3 Megabase deletion in the Xq25 region , encompassing the SH2D1A gene , was defined by SNP array genotyping .
	manualset3
112836	4	402247	13	NULL	NULL	0	NULL	SNP array genotyping	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A 3 Megabase deletion in the Xq25 region , encompassing the SH2D1A gene , was defined by SNP array genotyping .
	manualset3
112837	1	402248	13	NULL	NULL	0	NULL	Left ventricular volumes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Left ventricular volumes and pressure were ( mean + / - SD ) : ( SEE ARTICLE ) .
	manualset3
112838	2	402248	13	NULL	NULL	0	NULL	Left ventricular pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Left ventricular volumes and pressure were ( mean + / - SD ) : ( SEE ARTICLE ) .
	manualset3
112839	3	402248	13	NULL	NULL	0	NULL	mean + / - SD	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Left ventricular volumes and pressure were ( mean + / - SD ) : ( SEE ARTICLE ) .
	manualset3
112840	4	402248	13	NULL	NULL	0	NULL	ARTICLE	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Left ventricular volumes and pressure were ( mean + / - SD ) : ( SEE ARTICLE ) .
	manualset3
112841	1	402249	13	NULL	NULL	0	NULL	Leg 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Leg arteriopoplitealvenous differences of free fatty acids ( FFA ) showed an inverse intergroup relationship to that of glucose .
	manualset3
112842	2	402249	13	NULL	NULL	0	NULL	arteriopoplitealvenous differences	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Leg arteriopoplitealvenous differences of free fatty acids ( FFA ) showed an inverse intergroup relationship to that of glucose .
	manualset3
112843	3	402249	13	NULL	NULL	NULL	NULL	free fatty acids ( FFA )	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Leg arteriopoplitealvenous differences of free fatty acids ( FFA ) showed an inverse intergroup relationship to that of glucose .
	manualset3
112844	4	402249	13	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Leg arteriopoplitealvenous differences of free fatty acids ( FFA ) showed an inverse intergroup relationship to that of glucose .
	manualset3
112845	5	402249	13	NULL	NULL	0	NULL	glucose	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Leg arteriopoplitealvenous differences of free fatty acids ( FFA ) showed an inverse intergroup relationship to that of glucose .
	manualset3
112846	1	402250	13	NULL	NULL	0	NULL	Leiomyoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Leiomyoma of the esophagus ) .
	manualset3
112847	2	402250	13	NULL	NULL	0	NULL	esophagus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Leiomyoma of the esophagus ) .
	manualset3
112848	1	402251	13	NULL	NULL	0	NULL	Leiomyosarcoma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Leiomyosarcoma of the mediastinum is sufficiently rare ; therefore therapeutic approaches are not well defined .
	manualset3
112849	2	402251	13	NULL	NULL	0	NULL	mediastinum 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Leiomyosarcoma of the mediastinum is sufficiently rare ; therefore therapeutic approaches are not well defined .
	manualset3
112850	3	402251	13	NULL	NULL	0	NULL	therapeutic approaches	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Leiomyosarcoma of the mediastinum is sufficiently rare ; therefore therapeutic approaches are not well defined .
	manualset3
112851	1	402252	13	NULL	NULL	0	NULL	Lens 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Lens induces glaucoma -- a clinical study .
	manualset3
112852	2	402252	13	NULL	NULL	0	NULL	 glaucoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lens induces glaucoma -- a clinical study .
	manualset3
112853	3	402252	13	NULL	NULL	0	NULL	clinical study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Lens induces glaucoma -- a clinical study .
	manualset3
112854	1	402253	13	NULL	NULL	0	NULL	30 -fold increase	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A 30 - to 70-fold increase in the number of developing fat cells was achieved by the addition of cortisol or related corticosteroids in the presence of insulin .
	manualset3
112855	2	402253	13	NULL	NULL	0	NULL	70-fold increase	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A 30 - to 70-fold increase in the number of developing fat cells was achieved by the addition of cortisol or related corticosteroids in the presence of insulin .
	manualset3
112856	3	402253	13	NULL	NULL	0	NULL	fat cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A 30 - to 70-fold increase in the number of developing fat cells was achieved by the addition of cortisol or related corticosteroids in the presence of insulin .
	manualset3
112857	4	402253	13	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A 30 - to 70-fold increase in the number of developing fat cells was achieved by the addition of cortisol or related corticosteroids in the presence of insulin .
	manualset3
112858	5	402253	13	NULL	NULL	0	NULL	cortisol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A 30 - to 70-fold increase in the number of developing fat cells was achieved by the addition of cortisol or related corticosteroids in the presence of insulin .
	manualset3
112859	6	402253	13	NULL	NULL	0	NULL	corticosteroids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A 30 - to 70-fold increase in the number of developing fat cells was achieved by the addition of cortisol or related corticosteroids in the presence of insulin .
	manualset3
112860	7	402253	13	NULL	NULL	0	NULL	presence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 30 - to 70-fold increase in the number of developing fat cells was achieved by the addition of cortisol or related corticosteroids in the presence of insulin .
	manualset3
112861	8	402253	13	NULL	NULL	0	NULL	insulin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A 30 - to 70-fold increase in the number of developing fat cells was achieved by the addition of cortisol or related corticosteroids in the presence of insulin .
	manualset3
112862	1	402254	13	NULL	NULL	0	NULL	Lenticular card 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Lenticular card : a new method for denture identification .
	manualset3
112863	2	402254	13	NULL	NULL	0	NULL	method	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Lenticular card : a new method for denture identification .
	manualset3
112864	3	402254	13	NULL	NULL	0	NULL	denture identification	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Lenticular card : a new method for denture identification .
	manualset3
112865	1	402255	13	NULL	NULL	0	NULL	Leptin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Leptin treatment had no effect on plasma lipid profile and glucose level .
	manualset3
112866	2	402255	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Leptin treatment had no effect on plasma lipid profile and glucose level .
	manualset3
112867	3	402255	13	NULL	NULL	0	NULL	effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Leptin treatment had no effect on plasma lipid profile and glucose level .
	manualset3
112868	4	402255	13	NULL	NULL	0	NULL	plasma lipid profile	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Leptin treatment had no effect on plasma lipid profile and glucose level .
	manualset3
112869	5	402255	13	NULL	NULL	0	NULL	glucose level	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Leptin treatment had no effect on plasma lipid profile and glucose level .
	manualset3
112870	1	402256	13	NULL	NULL	0	NULL	Leptospiral antigens	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Leptospiral antigens ( L. interrogans serogroup ictero-haemorrhagiae ) in the kidney of experimentally infected guinea pigs and their relation to the pathogenesis of the renal injury .
	manualset3
112871	2	402256	13	NULL	NULL	0	NULL	L. interrogans serogroup ictero-haemorrhagiae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Leptospiral antigens ( L. interrogans serogroup ictero-haemorrhagiae ) in the kidney of experimentally infected guinea pigs and their relation to the pathogenesis of the renal injury .
	manualset3
112872	3	402256	13	NULL	NULL	0	NULL	kidney	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Leptospiral antigens ( L. interrogans serogroup ictero-haemorrhagiae ) in the kidney of experimentally infected guinea pigs and their relation to the pathogenesis of the renal injury .
	manualset3
112873	4	402256	13	NULL	NULL	0	NULL	guinea pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Leptospiral antigens ( L. interrogans serogroup ictero-haemorrhagiae ) in the kidney of experimentally infected guinea pigs and their relation to the pathogenesis of the renal injury .
	manualset3
112874	5	402256	13	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Leptospiral antigens ( L. interrogans serogroup ictero-haemorrhagiae ) in the kidney of experimentally infected guinea pigs and their relation to the pathogenesis of the renal injury .
	manualset3
112875	6	402256	13	NULL	NULL	0	NULL	pathogenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Leptospiral antigens ( L. interrogans serogroup ictero-haemorrhagiae ) in the kidney of experimentally infected guinea pigs and their relation to the pathogenesis of the renal injury .
	manualset3
112876	7	402256	13	NULL	NULL	0	NULL	renal injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Leptospiral antigens ( L. interrogans serogroup ictero-haemorrhagiae ) in the kidney of experimentally infected guinea pigs and their relation to the pathogenesis of the renal injury .
	manualset3
112877	1	402257	13	NULL	NULL	0	NULL	Leptospirosis-induced lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Leptospirosis-induced lesions , predominantly in the proximal tubule , were responsible for the polyuria and natriuresis observed .
	manualset3
112878	2	402257	13	NULL	NULL	0	NULL	proximal tubule	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Leptospirosis-induced lesions , predominantly in the proximal tubule , were responsible for the polyuria and natriuresis observed .
	manualset3
112879	3	402257	13	NULL	NULL	0	NULL	polyuria 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Leptospirosis-induced lesions , predominantly in the proximal tubule , were responsible for the polyuria and natriuresis observed .
	manualset3
112880	4	402257	13	NULL	NULL	0	NULL	natriuresis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Leptospirosis-induced lesions , predominantly in the proximal tubule , were responsible for the polyuria and natriuresis observed .
	manualset3
112881	1	402258	13	NULL	NULL	0	NULL	Leptospirosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Leptospirosis , a disease that is often under - or misdiagnosed , significantly impacts human health in many parts of the world and generally affects the most vulnerable communities .
	manualset3
112882	2	402258	13	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Leptospirosis , a disease that is often under - or misdiagnosed , significantly impacts human health in many parts of the world and generally affects the most vulnerable communities .
	manualset3
112883	3	402258	13	NULL	NULL	NULL	NULL	human health	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Leptospirosis , a disease that is often under - or misdiagnosed , significantly impacts human health in many parts of the world and generally affects the most vulnerable communities .
	manualset3
112884	4	402258	13	NULL	NULL	0	NULL	many parts	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Leptospirosis , a disease that is often under - or misdiagnosed , significantly impacts human health in many parts of the world and generally affects the most vulnerable communities .
	manualset3
112885	5	402258	13	NULL	NULL	0	NULL	world 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Leptospirosis , a disease that is often under - or misdiagnosed , significantly impacts human health in many parts of the world and generally affects the most vulnerable communities .
	manualset3
112886	6	402258	13	NULL	NULL	0	NULL	vulnerable communities	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Leptospirosis , a disease that is often under - or misdiagnosed , significantly impacts human health in many parts of the world and generally affects the most vulnerable communities .
	manualset3
112887	1	402259	13	NULL	NULL	0	NULL	dimensions	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Les dimensions affectives de l'engagement organisationnel et la satisfaction relative l'emploi sont considres d'importants lments prdictifs de l'intention de quitter , de l'absentisme et du rendement des travailleurs .
	manualset3
112888	1	402260	13	NULL	NULL	0	NULL	Lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions in nine patients were embolized with Polyvinyl Alcohol Particles ( PVA ) : this helped to stabilize the situation but could not avoid recurrences in all patients , necessitating complementary embolizations and or surgery .
	manualset3
112889	2	402260	13	NULL	NULL	0	NULL	nine patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions in nine patients were embolized with Polyvinyl Alcohol Particles ( PVA ) : this helped to stabilize the situation but could not avoid recurrences in all patients , necessitating complementary embolizations and or surgery .
	manualset3
112890	3	402260	13	NULL	NULL	0	NULL	Polyvinyl Alcohol Particles ( PVA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions in nine patients were embolized with Polyvinyl Alcohol Particles ( PVA ) : this helped to stabilize the situation but could not avoid recurrences in all patients , necessitating complementary embolizations and or surgery .
	manualset3
112891	4	402260	13	NULL	NULL	0	NULL	situation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions in nine patients were embolized with Polyvinyl Alcohol Particles ( PVA ) : this helped to stabilize the situation but could not avoid recurrences in all patients , necessitating complementary embolizations and or surgery .
	manualset3
112892	5	402260	13	NULL	NULL	0	NULL	recurrences	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions in nine patients were embolized with Polyvinyl Alcohol Particles ( PVA ) : this helped to stabilize the situation but could not avoid recurrences in all patients , necessitating complementary embolizations and or surgery .
	manualset3
112893	6	402260	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions in nine patients were embolized with Polyvinyl Alcohol Particles ( PVA ) : this helped to stabilize the situation but could not avoid recurrences in all patients , necessitating complementary embolizations and or surgery .
	manualset3
112894	7	402260	13	NULL	NULL	0	NULL	complementary embolizations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions in nine patients were embolized with Polyvinyl Alcohol Particles ( PVA ) : this helped to stabilize the situation but could not avoid recurrences in all patients , necessitating complementary embolizations and or surgery .
	manualset3
112895	8	402260	13	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions in nine patients were embolized with Polyvinyl Alcohol Particles ( PVA ) : this helped to stabilize the situation but could not avoid recurrences in all patients , necessitating complementary embolizations and or surgery .
	manualset3
112896	1	402261	13	NULL	NULL	0	NULL	Lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions in the nervous system are nearly always accompanied by cutaneous anomalies .
	manualset3
112897	2	402261	13	NULL	NULL	0	NULL	nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions in the nervous system are nearly always accompanied by cutaneous anomalies .
	manualset3
112898	3	402261	13	NULL	NULL	0	NULL	cutaneous anomalies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions in the nervous system are nearly always accompanied by cutaneous anomalies .
	manualset3
112899	1	402262	13	NULL	NULL	0	NULL	Lesions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions in the ovaries , uterus , and vagina may seriously influence normal reproductive capacity of dogs and cats and may put at risk the general health of the patients .
	manualset3
112900	2	402262	13	NULL	NULL	0	NULL	ovaries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions in the ovaries , uterus , and vagina may seriously influence normal reproductive capacity of dogs and cats and may put at risk the general health of the patients .
	manualset3
112901	3	402262	13	NULL	NULL	0	NULL	uterus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions in the ovaries , uterus , and vagina may seriously influence normal reproductive capacity of dogs and cats and may put at risk the general health of the patients .
	manualset3
112902	4	402262	13	NULL	NULL	0	NULL	vagina	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions in the ovaries , uterus , and vagina may seriously influence normal reproductive capacity of dogs and cats and may put at risk the general health of the patients .
	manualset3
112903	5	402262	13	NULL	NULL	0	NULL	reproductive capacity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions in the ovaries , uterus , and vagina may seriously influence normal reproductive capacity of dogs and cats and may put at risk the general health of the patients .
	manualset3
112904	6	402262	13	NULL	NULL	0	NULL	dogs 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions in the ovaries , uterus , and vagina may seriously influence normal reproductive capacity of dogs and cats and may put at risk the general health of the patients .
	manualset3
112905	7	402262	13	NULL	NULL	0	NULL	cats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions in the ovaries , uterus , and vagina may seriously influence normal reproductive capacity of dogs and cats and may put at risk the general health of the patients .
	manualset3
112906	8	402262	13	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions in the ovaries , uterus , and vagina may seriously influence normal reproductive capacity of dogs and cats and may put at risk the general health of the patients .
	manualset3
112907	9	402262	13	NULL	NULL	0	NULL	general health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions in the ovaries , uterus , and vagina may seriously influence normal reproductive capacity of dogs and cats and may put at risk the general health of the patients .
	manualset3
112908	10	402262	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions in the ovaries , uterus , and vagina may seriously influence normal reproductive capacity of dogs and cats and may put at risk the general health of the patients .
	manualset3
112909	1	402263	13	NULL	NULL	0	NULL	Lesions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions of the MLF -- internuclear ophthalmoparesis ( INO ) -- cause horizontal saccades to become disjunctive : adducting saccades are slow , small , or absent .
	manualset3
112910	2	402263	13	NULL	NULL	0	NULL	MLF	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions of the MLF -- internuclear ophthalmoparesis ( INO ) -- cause horizontal saccades to become disjunctive : adducting saccades are slow , small , or absent .
	manualset3
112911	3	402263	13	NULL	NULL	0	NULL	internuclear ophthalmoparesis ( INO ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions of the MLF -- internuclear ophthalmoparesis ( INO ) -- cause horizontal saccades to become disjunctive : adducting saccades are slow , small , or absent .
	manualset3
112912	4	402263	13	NULL	NULL	0	NULL	cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions of the MLF -- internuclear ophthalmoparesis ( INO ) -- cause horizontal saccades to become disjunctive : adducting saccades are slow , small , or absent .
	manualset3
112913	5	402263	13	NULL	NULL	0	NULL	horizontal saccades 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions of the MLF -- internuclear ophthalmoparesis ( INO ) -- cause horizontal saccades to become disjunctive : adducting saccades are slow , small , or absent .
	manualset3
112914	6	402263	13	NULL	NULL	0	NULL	saccades	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions of the MLF -- internuclear ophthalmoparesis ( INO ) -- cause horizontal saccades to become disjunctive : adducting saccades are slow , small , or absent .
	manualset3
112915	1	402264	13	NULL	NULL	0	NULL	Lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions of the breast associated with discharge from the nipple .
	manualset3
112916	2	402264	13	NULL	NULL	0	NULL	breast	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions of the breast associated with discharge from the nipple .
	manualset3
112917	3	402264	13	NULL	NULL	0	NULL	discharge	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions of the breast associated with discharge from the nipple .
	manualset3
112918	4	402264	13	NULL	NULL	0	NULL	nipple 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions of the breast associated with discharge from the nipple .
	manualset3
112919	1	402265	13	NULL	NULL	0	NULL	STAT1 methylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Less STAT1 methylation and subsequent increased STAT1-PIAS1 interaction are involved in the mechanism of the IFN-alpha-antagonistic activity of HBV .
	manualset3
112920	2	402265	13	NULL	NULL	0	NULL	STAT1-PIAS1 interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Less STAT1 methylation and subsequent increased STAT1-PIAS1 interaction are involved in the mechanism of the IFN-alpha-antagonistic activity of HBV .
	manualset3
112921	3	402265	13	NULL	NULL	0	NULL	mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Less STAT1 methylation and subsequent increased STAT1-PIAS1 interaction are involved in the mechanism of the IFN-alpha-antagonistic activity of HBV .
	manualset3
112922	4	402265	13	NULL	NULL	0	NULL	IFN-alpha-antagonistic activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Less STAT1 methylation and subsequent increased STAT1-PIAS1 interaction are involved in the mechanism of the IFN-alpha-antagonistic activity of HBV .
	manualset3
112923	5	402265	13	NULL	NULL	0	NULL	HBV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Less STAT1 methylation and subsequent increased STAT1-PIAS1 interaction are involved in the mechanism of the IFN-alpha-antagonistic activity of HBV .
	manualset3
112924	1	402266	13	NULL	NULL	0	NULL	Less eye movements	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Less eye movements were found for spatial and for easy questions .
	manualset3
112925	2	402266	13	NULL	NULL	0	NULL	questions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Less eye movements were found for spatial and for easy questions .
	manualset3
112926	1	402267	13	NULL	NULL	NULL	NULL	order of magnitude	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Less than one order of magnitude cell number reduction was also observed for suspensions of E. coli 10 ( 8 ) cells/mL and 0.002 mg/mL of TiO ( 2 ) .
	manualset3
112927	2	402267	13	NULL	NULL	0	NULL	cell number reduction	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Less than one order of magnitude cell number reduction was also observed for suspensions of E. coli 10 ( 8 ) cells/mL and 0.002 mg/mL of TiO ( 2 ) .
	manualset3
112928	3	402267	13	NULL	NULL	0	NULL	suspensions 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Less than one order of magnitude cell number reduction was also observed for suspensions of E. coli 10 ( 8 ) cells/mL and 0.002 mg/mL of TiO ( 2 ) .
	manualset3
112929	4	402267	13	NULL	NULL	0	NULL	E. coli 10 ( 8 ) cells/mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Less than one order of magnitude cell number reduction was also observed for suspensions of E. coli 10 ( 8 ) cells/mL and 0.002 mg/mL of TiO ( 2 ) .
	manualset3
112930	5	402267	13	NULL	NULL	0	NULL	0.002 mg/mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Less than one order of magnitude cell number reduction was also observed for suspensions of E. coli 10 ( 8 ) cells/mL and 0.002 mg/mL of TiO ( 2 ) .
	manualset3
112931	6	402267	13	NULL	NULL	0	NULL	TiO ( 2 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Less than one order of magnitude cell number reduction was also observed for suspensions of E. coli 10 ( 8 ) cells/mL and 0.002 mg/mL of TiO ( 2 ) .
	manualset3
112932	1	402268	13	NULL	NULL	0	NULL	angiographic findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Less common angiographic findings in this series consisted of segmental fusiform dilation of the artery , and lesions in the form of a septum that extended across the lumen .
	manualset3
112933	2	402268	13	NULL	NULL	0	NULL	series	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Less common angiographic findings in this series consisted of segmental fusiform dilation of the artery , and lesions in the form of a septum that extended across the lumen .
	manualset3
112934	3	402268	13	NULL	NULL	NULL	NULL	dilation of the artery	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Less common angiographic findings in this series consisted of segmental fusiform dilation of the artery , and lesions in the form of a septum that extended across the lumen .
	manualset3
112935	4	402268	13	NULL	NULL	0	NULL	lesions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Less common angiographic findings in this series consisted of segmental fusiform dilation of the artery , and lesions in the form of a septum that extended across the lumen .
	manualset3
112936	5	402268	13	NULL	NULL	0	NULL	form of a septum	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Less common angiographic findings in this series consisted of segmental fusiform dilation of the artery , and lesions in the form of a septum that extended across the lumen .
	manualset3
112937	6	402268	13	NULL	NULL	0	NULL	lumen 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Less common angiographic findings in this series consisted of segmental fusiform dilation of the artery , and lesions in the form of a septum that extended across the lumen .
	manualset3
112938	1	402269	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Less extensive data suggest that expression of the sex factor genes of an R factor of the N incompatibility group differs far less between E. coli and P. mirabilis hosts .
	manualset3
112939	2	402269	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Less extensive data suggest that expression of the sex factor genes of an R factor of the N incompatibility group differs far less between E. coli and P. mirabilis hosts .
	manualset3
112940	3	402269	13	NULL	NULL	0	NULL	sex factor genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Less extensive data suggest that expression of the sex factor genes of an R factor of the N incompatibility group differs far less between E. coli and P. mirabilis hosts .
	manualset3
112941	4	402269	13	NULL	NULL	0	NULL	R factor 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Less extensive data suggest that expression of the sex factor genes of an R factor of the N incompatibility group differs far less between E. coli and P. mirabilis hosts .
	manualset3
112942	5	402269	13	NULL	NULL	0	NULL	N incompatibility group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Less extensive data suggest that expression of the sex factor genes of an R factor of the N incompatibility group differs far less between E. coli and P. mirabilis hosts .
	manualset3
112943	6	402269	13	NULL	NULL	0	NULL	E. coli hosts 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Less extensive data suggest that expression of the sex factor genes of an R factor of the N incompatibility group differs far less between E. coli and P. mirabilis hosts .
	manualset3
112944	7	402269	13	NULL	NULL	0	NULL	P. mirabilis hosts 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Less extensive data suggest that expression of the sex factor genes of an R factor of the N incompatibility group differs far less between E. coli and P. mirabilis hosts .
	manualset3
112945	1	402270	13	NULL	NULL	0	NULL	33-year-old man	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A 33-year-old man was admitted because of jaundice .
	manualset3
112946	2	402270	13	NULL	NULL	0	NULL	jaundice	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 33-year-old man was admitted because of jaundice .
	manualset3
112947	1	402271	13	NULL	NULL	0	NULL	Lethal damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lethal damage caused by mild hyperthermia at 41.0 C or 42.0 C in both cell lines resulted in a low level of thermosensitivity , while sequential combination with PTL showed significant thermosensitization .
	manualset3
112948	2	402271	13	NULL	NULL	0	NULL	mild hyperthermia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lethal damage caused by mild hyperthermia at 41.0 C or 42.0 C in both cell lines resulted in a low level of thermosensitivity , while sequential combination with PTL showed significant thermosensitization .
	manualset3
112949	3	402271	13	NULL	NULL	0	NULL	41.0 C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Lethal damage caused by mild hyperthermia at 41.0 C or 42.0 C in both cell lines resulted in a low level of thermosensitivity , while sequential combination with PTL showed significant thermosensitization .
	manualset3
112950	4	402271	13	NULL	NULL	0	NULL	42.0 C 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Lethal damage caused by mild hyperthermia at 41.0 C or 42.0 C in both cell lines resulted in a low level of thermosensitivity , while sequential combination with PTL showed significant thermosensitization .
	manualset3
112951	5	402271	13	NULL	NULL	0	NULL	cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Lethal damage caused by mild hyperthermia at 41.0 C or 42.0 C in both cell lines resulted in a low level of thermosensitivity , while sequential combination with PTL showed significant thermosensitization .
	manualset3
112952	6	402271	13	NULL	NULL	0	NULL	low level of thermosensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lethal damage caused by mild hyperthermia at 41.0 C or 42.0 C in both cell lines resulted in a low level of thermosensitivity , while sequential combination with PTL showed significant thermosensitization .
	manualset3
112953	7	402271	13	NULL	NULL	0	NULL	sequential combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Lethal damage caused by mild hyperthermia at 41.0 C or 42.0 C in both cell lines resulted in a low level of thermosensitivity , while sequential combination with PTL showed significant thermosensitization .
	manualset3
112954	8	402271	13	NULL	NULL	0	NULL	PTL 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lethal damage caused by mild hyperthermia at 41.0 C or 42.0 C in both cell lines resulted in a low level of thermosensitivity , while sequential combination with PTL showed significant thermosensitization .
	manualset3
112955	9	402271	13	NULL	NULL	0	NULL	thermosensitization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lethal damage caused by mild hyperthermia at 41.0 C or 42.0 C in both cell lines resulted in a low level of thermosensitivity , while sequential combination with PTL showed significant thermosensitization .
	manualset3
112956	1	402272	13	NULL	NULL	0	NULL	Letter	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter : Acid-base changes during treatment of diabetic ketoacidosis .
	manualset3
112957	2	402272	13	NULL	NULL	0	NULL	Acid-base changes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter : Acid-base changes during treatment of diabetic ketoacidosis .
	manualset3
112958	3	402272	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter : Acid-base changes during treatment of diabetic ketoacidosis .
	manualset3
112959	4	402272	13	NULL	NULL	0	NULL	diabetic ketoacidosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter : Acid-base changes during treatment of diabetic ketoacidosis .
	manualset3
112960	1	402273	13	NULL	NULL	0	NULL	Letter	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter : Feeding and milk fever .
	manualset3
112961	2	402273	13	NULL	NULL	0	NULL	Feeding 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter : Feeding and milk fever .
	manualset3
112962	3	402273	13	NULL	NULL	0	NULL	milk fever	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter : Feeding and milk fever .
	manualset3
112963	1	402274	13	NULL	NULL	0	NULL	Letter	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter : Fixation devices and neoplastic changes in bone .
	manualset3
112964	2	402274	13	NULL	NULL	0	NULL	Fixation devices	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter : Fixation devices and neoplastic changes in bone .
	manualset3
112965	3	402274	13	NULL	NULL	0	NULL	neoplastic changes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter : Fixation devices and neoplastic changes in bone .
	manualset3
112966	4	402274	13	NULL	NULL	0	NULL	bone	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter : Fixation devices and neoplastic changes in bone .
	manualset3
112968	1	402275	13	NULL	NULL	0	NULL	Letter	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter : Potential carcinogenicity of iron dextran .
	manualset3
112969	2	402275	13	NULL	NULL	0	NULL	 Potential carcinogenicity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter : Potential carcinogenicity of iron dextran .
	manualset3
112970	3	402275	13	NULL	NULL	0	NULL	iron dextran	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter : Potential carcinogenicity of iron dextran .
	manualset3
112985	1	402276	13	NULL	NULL	0	NULL	Letter	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter : Quality care threatened by PL 93-641 .
	manualset3
112986	2	402276	13	NULL	NULL	0	NULL	Quality care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter : Quality care threatened by PL 93-641 .
	manualset3
112987	3	402276	13	NULL	NULL	0	NULL	PL 93-641	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter : Quality care threatened by PL 93-641 .
	manualset3
112988	1	402277	13	NULL	NULL	0	NULL	34-year-old female patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A 34-year-old female patient underwent living donor liver transplantation for Budd-Chiari syndrome .
	manualset3
112989	2	402277	13	NULL	NULL	0	NULL	liver transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A 34-year-old female patient underwent living donor liver transplantation for Budd-Chiari syndrome .
	manualset3
112991	3	402277	13	NULL	NULL	0	NULL	Budd-Chiari syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A 34-year-old female patient underwent living donor liver transplantation for Budd-Chiari syndrome .
	manualset3
112992	1	402278	13	NULL	NULL	0	NULL	Letter	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter : Results of radiation treatment of primary mammary carcinoma .
	manualset3
112993	2	402278	13	NULL	NULL	0	NULL	Results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter : Results of radiation treatment of primary mammary carcinoma .
	manualset3
112994	3	402278	13	NULL	NULL	0	NULL	radiation treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter : Results of radiation treatment of primary mammary carcinoma .
	manualset3
112995	4	402278	13	NULL	NULL	0	NULL	 primary mammary carcinoma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter : Results of radiation treatment of primary mammary carcinoma .
	manualset3
112996	1	402279	13	NULL	NULL	0	NULL	Letter	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter : Should liver scan be a prerequisite to liver biopsy ?
	manualset3
112997	2	402279	13	NULL	NULL	0	NULL	liver scan	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter : Should liver scan be a prerequisite to liver biopsy ?
	manualset3
112998	3	402279	13	NULL	NULL	0	NULL	prerequisite	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter : Should liver scan be a prerequisite to liver biopsy ?
	manualset3
112999	4	402279	13	NULL	NULL	0	NULL	liver biopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter : Should liver scan be a prerequisite to liver biopsy ?
	manualset3
113000	1	402280	13	NULL	NULL	0	NULL	Letter	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter : abortion ( Amendment ) Bill .
	manualset3
113001	2	402280	13	NULL	NULL	0	NULL	 abortion ( Amendment ) Bill	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter : abortion ( Amendment ) Bill .
	manualset3
113002	1	402281	13	NULL	NULL	0	NULL	Letter	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter by Sengupta et al regarding article , `` Mechanisms of preejection and postejection velocity spikes in left ventricular myocardium : interaction between wall deformation and valve events '' .
	manualset3
113003	2	402281	13	NULL	NULL	0	NULL	Sengupta et al	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter by Sengupta et al regarding article , `` Mechanisms of preejection and postejection velocity spikes in left ventricular myocardium : interaction between wall deformation and valve events '' .
	manualset3
113004	3	402281	13	NULL	NULL	0	NULL	article 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter by Sengupta et al regarding article , `` Mechanisms of preejection and postejection velocity spikes in left ventricular myocardium : interaction between wall deformation and valve events '' .
	manualset3
113005	4	402281	13	NULL	NULL	0	NULL	Mechanisms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter by Sengupta et al regarding article , `` Mechanisms of preejection and postejection velocity spikes in left ventricular myocardium : interaction between wall deformation and valve events '' .
	manualset3
113006	5	402281	13	NULL	NULL	0	NULL	preejection velocity spikes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter by Sengupta et al regarding article , `` Mechanisms of preejection and postejection velocity spikes in left ventricular myocardium : interaction between wall deformation and valve events '' .
	manualset3
113007	6	402281	13	NULL	NULL	0	NULL	postejection velocity spikes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter by Sengupta et al regarding article , `` Mechanisms of preejection and postejection velocity spikes in left ventricular myocardium : interaction between wall deformation and valve events '' .
	manualset3
113008	7	402281	13	NULL	NULL	0	NULL	left ventricular myocardium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter by Sengupta et al regarding article , `` Mechanisms of preejection and postejection velocity spikes in left ventricular myocardium : interaction between wall deformation and valve events '' .
	manualset3
113009	8	402281	13	NULL	NULL	0	NULL	interaction 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter by Sengupta et al regarding article , `` Mechanisms of preejection and postejection velocity spikes in left ventricular myocardium : interaction between wall deformation and valve events '' .
	manualset3
113010	9	402281	13	NULL	NULL	0	NULL	wall deformation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter by Sengupta et al regarding article , `` Mechanisms of preejection and postejection velocity spikes in left ventricular myocardium : interaction between wall deformation and valve events '' .
	manualset3
113011	10	402281	13	NULL	NULL	0	NULL	valve events	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter by Sengupta et al regarding article , `` Mechanisms of preejection and postejection velocity spikes in left ventricular myocardium : interaction between wall deformation and valve events '' .
	manualset3
113012	1	402282	13	NULL	NULL	0	NULL	Letter 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter from the ASHI president and council .
	manualset3
113013	2	402282	13	NULL	NULL	0	NULL	ASHI president	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter from the ASHI president and council .
	manualset3
113014	3	402282	13	NULL	NULL	0	NULL	council	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Letter from the ASHI president and council .
	manualset3
113015	1	402283	13	NULL	NULL	0	NULL	Leucine zipper-mediated homodimerization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Leucine zipper-mediated homodimerization of the p21-activated kinase-interacting factor , beta Pix .
	manualset3
113016	2	402283	13	NULL	NULL	0	NULL	p21-activated kinase-interacting factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Leucine zipper-mediated homodimerization of the p21-activated kinase-interacting factor , beta Pix .
	manualset3
113017	3	402283	13	NULL	NULL	0	NULL	beta Pix	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Leucine zipper-mediated homodimerization of the p21-activated kinase-interacting factor , beta Pix .
	manualset3
113018	1	402284	13	NULL	NULL	0	NULL	Leucocyte cation transport	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Leucocyte cation transport measured when patients received a normal sodium intake and the response of the renin-angiotensin system to changes in sodium intake were studied in 22 patients with essential hypertension .
	manualset3
113019	2	402284	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Leucocyte cation transport measured when patients received a normal sodium intake and the response of the renin-angiotensin system to changes in sodium intake were studied in 22 patients with essential hypertension .
	manualset3
113020	3	402284	13	NULL	NULL	0	NULL	sodium intake 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Leucocyte cation transport measured when patients received a normal sodium intake and the response of the renin-angiotensin system to changes in sodium intake were studied in 22 patients with essential hypertension .
	manualset3
113021	4	402284	13	NULL	NULL	0	NULL	response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Leucocyte cation transport measured when patients received a normal sodium intake and the response of the renin-angiotensin system to changes in sodium intake were studied in 22 patients with essential hypertension .
	manualset3
113022	5	402284	13	NULL	NULL	0	NULL	renin-angiotensin system	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Leucocyte cation transport measured when patients received a normal sodium intake and the response of the renin-angiotensin system to changes in sodium intake were studied in 22 patients with essential hypertension .
	manualset3
113023	6	402284	13	NULL	NULL	0	NULL	changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Leucocyte cation transport measured when patients received a normal sodium intake and the response of the renin-angiotensin system to changes in sodium intake were studied in 22 patients with essential hypertension .
	manualset3
113024	7	402284	13	NULL	NULL	0	NULL	sodium intake 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Leucocyte cation transport measured when patients received a normal sodium intake and the response of the renin-angiotensin system to changes in sodium intake were studied in 22 patients with essential hypertension .
	manualset3
113025	8	402284	13	NULL	NULL	0	NULL	22 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Leucocyte cation transport measured when patients received a normal sodium intake and the response of the renin-angiotensin system to changes in sodium intake were studied in 22 patients with essential hypertension .
	manualset3
113026	9	402284	13	NULL	NULL	0	NULL	essential hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Leucocyte cation transport measured when patients received a normal sodium intake and the response of the renin-angiotensin system to changes in sodium intake were studied in 22 patients with essential hypertension .
	manualset3
113027	1	402285	13	NULL	NULL	0	NULL	Leukoneutropenia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Leukoneutropenia and thrombopenia are both exceptional .
	manualset3
113028	2	402285	13	NULL	NULL	0	NULL	thrombopenia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Leukoneutropenia and thrombopenia are both exceptional .
	manualset3
113029	1	402286	13	NULL	NULL	0	NULL	Leukotriene D4 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Leukotriene D4 increases both the force of contraction and polyphosphoinositide formation in guinea-pig papillary muscle .
	manualset3
113030	2	402286	13	NULL	NULL	0	NULL	increases	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Leukotriene D4 increases both the force of contraction and polyphosphoinositide formation in guinea-pig papillary muscle .
	manualset3
113031	3	402286	13	NULL	NULL	0	NULL	force of contraction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Leukotriene D4 increases both the force of contraction and polyphosphoinositide formation in guinea-pig papillary muscle .
	manualset3
113032	4	402286	13	NULL	NULL	0	NULL	polyphosphoinositide formation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Leukotriene D4 increases both the force of contraction and polyphosphoinositide formation in guinea-pig papillary muscle .
	manualset3
113033	5	402286	13	NULL	NULL	0	NULL	guinea-pig papillary muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Leukotriene D4 increases both the force of contraction and polyphosphoinositide formation in guinea-pig papillary muscle .
	manualset3
113034	1	402287	13	NULL	NULL	0	NULL	Level of Evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Level of Evidence : Level II , therapeutic study .
	manualset3
113035	2	402287	13	NULL	NULL	0	NULL	Level II	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Level of Evidence : Level II , therapeutic study .
	manualset3
113036	3	402287	13	NULL	NULL	0	NULL	 therapeutic study 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Level of Evidence : Level II , therapeutic study .
	manualset3
113037	1	402288	13	NULL	NULL	0	NULL	Level	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Level of bound metabolites was 1.5 times higher in the nasal mucosa than in the liver of the ( 2 ' -14 C ) NNN monkey .
	manualset3
113038	2	402288	13	NULL	NULL	0	NULL	metabolites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Level of bound metabolites was 1.5 times higher in the nasal mucosa than in the liver of the ( 2 ' -14 C ) NNN monkey .
	manualset3
113039	3	402288	13	NULL	NULL	0	NULL	1.5 times	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Level of bound metabolites was 1.5 times higher in the nasal mucosa than in the liver of the ( 2 ' -14 C ) NNN monkey .
	manualset3
113040	4	402288	13	NULL	NULL	0	NULL	nasal mucosa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Level of bound metabolites was 1.5 times higher in the nasal mucosa than in the liver of the ( 2 ' -14 C ) NNN monkey .
	manualset3
113041	5	402288	13	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Level of bound metabolites was 1.5 times higher in the nasal mucosa than in the liver of the ( 2 ' -14 C ) NNN monkey .
	manualset3
113042	6	402288	13	NULL	NULL	0	NULL	( 2 ' -14 C ) NNN monkey	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Level of bound metabolites was 1.5 times higher in the nasal mucosa than in the liver of the ( 2 ' -14 C ) NNN monkey .
	manualset3
113043	1	402289	13	NULL	NULL	0	NULL	Levels of 5-HT	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of 5-HT in the corpus striatum and the midbrain of males were greater than those of the female .
	manualset3
113044	2	402289	13	NULL	NULL	0	NULL	corpus striatum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of 5-HT in the corpus striatum and the midbrain of males were greater than those of the female .
	manualset3
113045	3	402289	13	NULL	NULL	0	NULL	midbrain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of 5-HT in the corpus striatum and the midbrain of males were greater than those of the female .
	manualset3
113046	4	402289	13	NULL	NULL	0	NULL	males	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of 5-HT in the corpus striatum and the midbrain of males were greater than those of the female .
	manualset3
113047	5	402289	13	NULL	NULL	0	NULL	female 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of 5-HT in the corpus striatum and the midbrain of males were greater than those of the female .
	manualset3
113048	1	402290	13	NULL	NULL	0	NULL	Levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of MCP-1 mRNA and protein were determined by Northern blot analysis and ELISA , respectively .
	manualset3
113049	2	402290	13	NULL	NULL	0	NULL	MCP-1 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of MCP-1 mRNA and protein were determined by Northern blot analysis and ELISA , respectively .
	manualset3
113050	3	402290	13	NULL	NULL	0	NULL	MCP-1 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of MCP-1 mRNA and protein were determined by Northern blot analysis and ELISA , respectively .
	manualset3
113051	4	402290	13	NULL	NULL	0	NULL	Northern blot analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of MCP-1 mRNA and protein were determined by Northern blot analysis and ELISA , respectively .
	manualset3
113052	5	402290	13	NULL	NULL	NULL	NULL	ELISA	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Levels of MCP-1 mRNA and protein were determined by Northern blot analysis and ELISA , respectively .
	manualset3
113053	1	402291	13	NULL	NULL	0	NULL	Levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of aP2 protein were still high , in some cases , 1 day after the decrease in mRNA levels consistent with a long half-life of the protein .
	manualset3
113054	2	402291	13	NULL	NULL	0	NULL	aP2 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of aP2 protein were still high , in some cases , 1 day after the decrease in mRNA levels consistent with a long half-life of the protein .
	manualset3
113055	3	402291	13	NULL	NULL	0	NULL	cases	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of aP2 protein were still high , in some cases , 1 day after the decrease in mRNA levels consistent with a long half-life of the protein .
	manualset3
113056	4	402291	13	NULL	NULL	0	NULL	1 day	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of aP2 protein were still high , in some cases , 1 day after the decrease in mRNA levels consistent with a long half-life of the protein .
	manualset3
113057	5	402291	13	NULL	NULL	0	NULL	decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of aP2 protein were still high , in some cases , 1 day after the decrease in mRNA levels consistent with a long half-life of the protein .
	manualset3
113058	6	402291	13	NULL	NULL	0	NULL	mRNA levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of aP2 protein were still high , in some cases , 1 day after the decrease in mRNA levels consistent with a long half-life of the protein .
	manualset3
113059	7	402291	13	NULL	NULL	0	NULL	long half-life	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of aP2 protein were still high , in some cases , 1 day after the decrease in mRNA levels consistent with a long half-life of the protein .
	manualset3
113060	8	402291	13	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of aP2 protein were still high , in some cases , 1 day after the decrease in mRNA levels consistent with a long half-life of the protein .
	manualset3
113061	1	402292	13	NULL	NULL	0	NULL	Levels of anxiety	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of anxiety were higher in the two groups with a confirmed diagnosis in the antenatal period or after birth ( 62 % ) than in those who were screened positively but in whom no abnormality was found ( 30 % ) ( p = 0.0055 ) .
	manualset3
113062	2	402292	13	NULL	NULL	0	NULL	two groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of anxiety were higher in the two groups with a confirmed diagnosis in the antenatal period or after birth ( 62 % ) than in those who were screened positively but in whom no abnormality was found ( 30 % ) ( p = 0.0055 ) .
	manualset3
113063	3	402292	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of anxiety were higher in the two groups with a confirmed diagnosis in the antenatal period or after birth ( 62 % ) than in those who were screened positively but in whom no abnormality was found ( 30 % ) ( p = 0.0055 ) .
	manualset3
113064	4	402292	13	NULL	NULL	0	NULL	antenatal period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of anxiety were higher in the two groups with a confirmed diagnosis in the antenatal period or after birth ( 62 % ) than in those who were screened positively but in whom no abnormality was found ( 30 % ) ( p = 0.0055 ) .
	manualset3
113065	5	402292	13	NULL	NULL	0	NULL	birth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of anxiety were higher in the two groups with a confirmed diagnosis in the antenatal period or after birth ( 62 % ) than in those who were screened positively but in whom no abnormality was found ( 30 % ) ( p = 0.0055 ) .
	manualset3
113066	6	402292	13	NULL	NULL	0	NULL	62 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of anxiety were higher in the two groups with a confirmed diagnosis in the antenatal period or after birth ( 62 % ) than in those who were screened positively but in whom no abnormality was found ( 30 % ) ( p = 0.0055 ) .
	manualset3
113067	7	402292	13	NULL	NULL	0	NULL	abnormality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of anxiety were higher in the two groups with a confirmed diagnosis in the antenatal period or after birth ( 62 % ) than in those who were screened positively but in whom no abnormality was found ( 30 % ) ( p = 0.0055 ) .
	manualset3
113068	8	402292	13	NULL	NULL	0	NULL	30 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of anxiety were higher in the two groups with a confirmed diagnosis in the antenatal period or after birth ( 62 % ) than in those who were screened positively but in whom no abnormality was found ( 30 % ) ( p = 0.0055 ) .
	manualset3
113069	9	402292	13	NULL	NULL	0	NULL	p = 0.0055	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of anxiety were higher in the two groups with a confirmed diagnosis in the antenatal period or after birth ( 62 % ) than in those who were screened positively but in whom no abnormality was found ( 30 % ) ( p = 0.0055 ) .
	manualset3
113070	1	402293	13	NULL	NULL	0	NULL	34 bp deletion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A 34 bp deletion within TSC2 is a rare polymorphism , not a pathogenic mutation .
	manualset3
113071	2	402293	13	NULL	NULL	0	NULL	TSC2	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A 34 bp deletion within TSC2 is a rare polymorphism , not a pathogenic mutation .
	manualset3
113072	3	402293	13	NULL	NULL	0	NULL	polymorphism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A 34 bp deletion within TSC2 is a rare polymorphism , not a pathogenic mutation .
	manualset3
113073	4	402293	13	NULL	NULL	0	NULL	pathogenic mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A 34 bp deletion within TSC2 is a rare polymorphism , not a pathogenic mutation .
	manualset3
113074	1	402294	13	NULL	NULL	0	NULL	Levels of circulating immune complexes ( CICs ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of circulating immune complexes ( CICs ) were increased ( greater than 11 % ( 125I ) C1q binding ) in 14 of the 20 men prior to treatment .
	manualset3
113075	2	402294	13	NULL	NULL	0	NULL	greater than 11 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of circulating immune complexes ( CICs ) were increased ( greater than 11 % ( 125I ) C1q binding ) in 14 of the 20 men prior to treatment .
	manualset3
113076	3	402294	13	NULL	NULL	0	NULL	( 125I ) C1q binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of circulating immune complexes ( CICs ) were increased ( greater than 11 % ( 125I ) C1q binding ) in 14 of the 20 men prior to treatment .
	manualset3
113077	4	402294	13	NULL	NULL	0	NULL	14 of the 20 men	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of circulating immune complexes ( CICs ) were increased ( greater than 11 % ( 125I ) C1q binding ) in 14 of the 20 men prior to treatment .
	manualset3
113078	5	402294	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of circulating immune complexes ( CICs ) were increased ( greater than 11 % ( 125I ) C1q binding ) in 14 of the 20 men prior to treatment .
	manualset3
113079	1	402295	13	NULL	NULL	0	NULL	Levels of protein C	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of protein C correlated with levels of factor VIII activity but did not correlate with markers of consumptive coagulopathy .
	manualset3
113080	2	402295	13	NULL	NULL	0	NULL	levels 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of protein C correlated with levels of factor VIII activity but did not correlate with markers of consumptive coagulopathy .
	manualset3
113081	3	402295	13	NULL	NULL	0	NULL	factor VIII activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of protein C correlated with levels of factor VIII activity but did not correlate with markers of consumptive coagulopathy .
	manualset3
113082	4	402295	13	NULL	NULL	0	NULL	markers	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of protein C correlated with levels of factor VIII activity but did not correlate with markers of consumptive coagulopathy .
	manualset3
113083	5	402295	13	NULL	NULL	0	NULL	consumptive coagulopathy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of protein C correlated with levels of factor VIII activity but did not correlate with markers of consumptive coagulopathy .
	manualset3
113084	1	402296	13	NULL	NULL	0	NULL	Lewis rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Lewis rats showed lower levels of class I MHC in the hypothalamic paraventricular nucleus ( PVN ) and retrochiasmatic area ( RCA ) compared to Fischer rats under both vehicle and LPS conditions .
	manualset3
113085	2	402296	13	NULL	NULL	0	NULL	levels of class I MHC	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Lewis rats showed lower levels of class I MHC in the hypothalamic paraventricular nucleus ( PVN ) and retrochiasmatic area ( RCA ) compared to Fischer rats under both vehicle and LPS conditions .
	manualset3
113086	3	402296	13	NULL	NULL	0	NULL	hypothalamic paraventricular nucleus ( PVN ) 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Lewis rats showed lower levels of class I MHC in the hypothalamic paraventricular nucleus ( PVN ) and retrochiasmatic area ( RCA ) compared to Fischer rats under both vehicle and LPS conditions .
	manualset3
113087	4	402296	13	NULL	NULL	0	NULL	retrochiasmatic area ( RCA )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Lewis rats showed lower levels of class I MHC in the hypothalamic paraventricular nucleus ( PVN ) and retrochiasmatic area ( RCA ) compared to Fischer rats under both vehicle and LPS conditions .
	manualset3
113088	5	402296	13	NULL	NULL	0	NULL	Fischer rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Lewis rats showed lower levels of class I MHC in the hypothalamic paraventricular nucleus ( PVN ) and retrochiasmatic area ( RCA ) compared to Fischer rats under both vehicle and LPS conditions .
	manualset3
113089	6	402296	13	NULL	NULL	0	NULL	vehicle	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Lewis rats showed lower levels of class I MHC in the hypothalamic paraventricular nucleus ( PVN ) and retrochiasmatic area ( RCA ) compared to Fischer rats under both vehicle and LPS conditions .
	manualset3
113090	7	402296	13	NULL	NULL	0	NULL	LPS conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Lewis rats showed lower levels of class I MHC in the hypothalamic paraventricular nucleus ( PVN ) and retrochiasmatic area ( RCA ) compared to Fischer rats under both vehicle and LPS conditions .
	manualset3
113091	1	402297	13	NULL	NULL	0	NULL	Li-Fraumeni syndrome ( LFS )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Li-Fraumeni syndrome ( LFS ) is an autosomal dominantly inherited disorder characterized by a strikingly increased risk of early-onset breast cancer , sarcomas , brain tumors and other neoplasms in individuals harboring germline TP53 mutations .
	manualset3
113092	2	402297	13	NULL	NULL	0	NULL	autosomal dominantly inherited disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Li-Fraumeni syndrome ( LFS ) is an autosomal dominantly inherited disorder characterized by a strikingly increased risk of early-onset breast cancer , sarcomas , brain tumors and other neoplasms in individuals harboring germline TP53 mutations .
	manualset3
113093	3	402297	13	NULL	NULL	0	NULL	risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Li-Fraumeni syndrome ( LFS ) is an autosomal dominantly inherited disorder characterized by a strikingly increased risk of early-onset breast cancer , sarcomas , brain tumors and other neoplasms in individuals harboring germline TP53 mutations .
	manualset3
113094	4	402297	13	NULL	NULL	0	NULL	early-onset breast cancer	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Li-Fraumeni syndrome ( LFS ) is an autosomal dominantly inherited disorder characterized by a strikingly increased risk of early-onset breast cancer , sarcomas , brain tumors and other neoplasms in individuals harboring germline TP53 mutations .
	manualset3
113095	5	402297	13	NULL	NULL	0	NULL	sarcomas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Li-Fraumeni syndrome ( LFS ) is an autosomal dominantly inherited disorder characterized by a strikingly increased risk of early-onset breast cancer , sarcomas , brain tumors and other neoplasms in individuals harboring germline TP53 mutations .
	manualset3
113096	6	402297	13	NULL	NULL	0	NULL	brain tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Li-Fraumeni syndrome ( LFS ) is an autosomal dominantly inherited disorder characterized by a strikingly increased risk of early-onset breast cancer , sarcomas , brain tumors and other neoplasms in individuals harboring germline TP53 mutations .
	manualset3
113097	7	402297	13	NULL	NULL	0	NULL	neoplasms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Li-Fraumeni syndrome ( LFS ) is an autosomal dominantly inherited disorder characterized by a strikingly increased risk of early-onset breast cancer , sarcomas , brain tumors and other neoplasms in individuals harboring germline TP53 mutations .
	manualset3
113098	8	402297	13	NULL	NULL	0	NULL	individuals 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Li-Fraumeni syndrome ( LFS ) is an autosomal dominantly inherited disorder characterized by a strikingly increased risk of early-onset breast cancer , sarcomas , brain tumors and other neoplasms in individuals harboring germline TP53 mutations .
	manualset3
113099	9	402297	13	NULL	NULL	0	NULL	germline TP53 mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Li-Fraumeni syndrome ( LFS ) is an autosomal dominantly inherited disorder characterized by a strikingly increased risk of early-onset breast cancer , sarcomas , brain tumors and other neoplasms in individuals harboring germline TP53 mutations .
	manualset3
113100	1	402298	13	NULL	NULL	0	NULL	Liberators	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Liberators of NO exert a dual effect on renin secretion from isolated mouse renal juxtaglomerular cells .
	manualset3
113101	2	402298	13	NULL	NULL	0	NULL	NO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Liberators of NO exert a dual effect on renin secretion from isolated mouse renal juxtaglomerular cells .
	manualset3
113102	3	402298	13	NULL	NULL	NULL	NULL	dual effect 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Liberators of NO exert a dual effect on renin secretion from isolated mouse renal juxtaglomerular cells .
	manualset3
113103	4	402298	13	NULL	NULL	0	NULL	renin secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Liberators of NO exert a dual effect on renin secretion from isolated mouse renal juxtaglomerular cells .
	manualset3
113104	5	402298	13	NULL	NULL	0	NULL	mouse renal juxtaglomerular cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Liberators of NO exert a dual effect on renin secretion from isolated mouse renal juxtaglomerular cells .
	manualset3
113105	1	402299	13	NULL	NULL	0	NULL	Lichen planus-like eruption	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lichen planus-like eruption following autologous bone marrow transplantation for chronic myeloid leukemia .
	manualset3
113106	2	402299	13	NULL	NULL	0	NULL	autologous bone marrow transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Lichen planus-like eruption following autologous bone marrow transplantation for chronic myeloid leukemia .
	manualset3
113107	3	402299	13	NULL	NULL	0	NULL	chronic myeloid leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Lichen planus-like eruption following autologous bone marrow transplantation for chronic myeloid leukemia .
	manualset3
113108	1	402300	13	NULL	NULL	0	NULL	36-year-old female	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A 36-year-old female was admitted with leptomeningeal melanoma associated with straight sinus thrombosis manifesting as headache and vomiting .
	manualset3
113109	2	402300	13	NULL	NULL	0	NULL	leptomeningeal melanoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A 36-year-old female was admitted with leptomeningeal melanoma associated with straight sinus thrombosis manifesting as headache and vomiting .
	manualset3
113110	3	402300	13	NULL	NULL	0	NULL	straight sinus thrombosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 36-year-old female was admitted with leptomeningeal melanoma associated with straight sinus thrombosis manifesting as headache and vomiting .
	manualset3
113111	4	402300	13	NULL	NULL	0	NULL	headache	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 36-year-old female was admitted with leptomeningeal melanoma associated with straight sinus thrombosis manifesting as headache and vomiting .
	manualset3
113112	5	402300	13	NULL	NULL	0	NULL	vomiting 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 36-year-old female was admitted with leptomeningeal melanoma associated with straight sinus thrombosis manifesting as headache and vomiting .
	manualset3
113113	1	402301	13	NULL	NULL	0	NULL	Life-threatening complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Life-threatening complications related to minocycline pleurodesis .
	manualset3
113114	2	402301	13	NULL	NULL	0	NULL	minocycline pleurodesis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Life-threatening complications related to minocycline pleurodesis .
	manualset3
113115	1	402302	13	NULL	NULL	0	NULL	Life history study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Life history study of the mite produced very novel and interesting results .
	manualset3
113116	2	402302	13	NULL	NULL	0	NULL	mite	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Life history study of the mite produced very novel and interesting results .
	manualset3
113117	3	402302	13	NULL	NULL	0	NULL	novel results	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Life history study of the mite produced very novel and interesting results .
	manualset3
113118	4	402302	13	NULL	NULL	0	NULL	interesting results 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Life history study of the mite produced very novel and interesting results .
	manualset3
113119	1	402303	13	NULL	NULL	0	NULL	Life support systems	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Life support systems represent one of the most critical aspects of human space exploration .
	manualset3
113120	2	402303	13	NULL	NULL	0	NULL	critical aspects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Life support systems represent one of the most critical aspects of human space exploration .
	manualset3
113121	3	402303	13	NULL	NULL	NULL	NULL	 human space exploration 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Life support systems represent one of the most critical aspects of human space exploration .
	manualset3
113140	1	402304	13	NULL	NULL	0	NULL	Life 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Life as a military doc commands attention .
	manualset3
113141	2	402304	13	NULL	NULL	0	NULL	military doc 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Life as a military doc commands attention .
	manualset3
113142	3	402304	13	NULL	NULL	0	NULL	commands	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Life as a military doc commands attention .
	manualset3
113143	4	402304	13	NULL	NULL	0	NULL	attention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Life as a military doc commands attention .
	manualset3
113144	1	402305	13	NULL	NULL	0	NULL	Lifetimes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lifetimes of photosystem I and II proteins in the cyanobacterium Synechocystis sp .
	manualset3
113145	2	402305	13	NULL	NULL	0	NULL	photosystem I proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Lifetimes of photosystem I and II proteins in the cyanobacterium Synechocystis sp .
	manualset3
113146	3	402305	13	NULL	NULL	0	NULL	photosystem II proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Lifetimes of photosystem I and II proteins in the cyanobacterium Synechocystis sp .
	manualset3
113147	4	402305	13	NULL	NULL	0	NULL	cyanobacterium Synechocystis sp	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Lifetimes of photosystem I and II proteins in the cyanobacterium Synechocystis sp .
	manualset3
113148	1	402306	13	NULL	NULL	0	NULL	Ligands 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ligands recognizing the minor groove of DNA : development and applications .
	manualset3
113149	2	402306	13	NULL	NULL	0	NULL	minor groove of DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Ligands recognizing the minor groove of DNA : development and applications .
	manualset3
113150	3	402306	13	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ligands recognizing the minor groove of DNA : development and applications .
	manualset3
113151	4	402306	13	NULL	NULL	0	NULL	applications 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ligands recognizing the minor groove of DNA : development and applications .
	manualset3
113152	1	402307	13	NULL	NULL	0	NULL	Light-brown apple moth larvae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Light-brown apple moth larvae fed with apple leaves expressing Na-PI had significantly reduced body weight after 7 days of feeding and female pupae were 19-28 % smaller than controls .
	manualset3
113153	2	402307	13	NULL	NULL	0	NULL	apple leaves 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Light-brown apple moth larvae fed with apple leaves expressing Na-PI had significantly reduced body weight after 7 days of feeding and female pupae were 19-28 % smaller than controls .
	manualset3
113154	3	402307	13	NULL	NULL	0	NULL	Na-PI 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Light-brown apple moth larvae fed with apple leaves expressing Na-PI had significantly reduced body weight after 7 days of feeding and female pupae were 19-28 % smaller than controls .
	manualset3
113155	4	402307	13	NULL	NULL	0	NULL	body weight	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Light-brown apple moth larvae fed with apple leaves expressing Na-PI had significantly reduced body weight after 7 days of feeding and female pupae were 19-28 % smaller than controls .
	manualset3
113156	5	402307	13	NULL	NULL	NULL	NULL	7 days 	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Light-brown apple moth larvae fed with apple leaves expressing Na-PI had significantly reduced body weight after 7 days of feeding and female pupae were 19-28 % smaller than controls .
	manualset3
113157	6	402307	13	NULL	NULL	0	NULL	feeding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Light-brown apple moth larvae fed with apple leaves expressing Na-PI had significantly reduced body weight after 7 days of feeding and female pupae were 19-28 % smaller than controls .
	manualset3
113158	7	402307	13	NULL	NULL	0	NULL	female pupae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Light-brown apple moth larvae fed with apple leaves expressing Na-PI had significantly reduced body weight after 7 days of feeding and female pupae were 19-28 % smaller than controls .
	manualset3
113159	8	402307	13	NULL	NULL	0	NULL	19-28 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Light-brown apple moth larvae fed with apple leaves expressing Na-PI had significantly reduced body weight after 7 days of feeding and female pupae were 19-28 % smaller than controls .
	manualset3
113160	9	402307	13	NULL	NULL	0	NULL	controls 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Light-brown apple moth larvae fed with apple leaves expressing Na-PI had significantly reduced body weight after 7 days of feeding and female pupae were 19-28 % smaller than controls .
	manualset3
113161	1	402308	13	NULL	NULL	0	NULL	induction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Light-dependent induction of cFos during subjective day and night in PACAP-containing ganglion cells of the retinohypothalamic tract .
	manualset3
113162	2	402308	13	NULL	NULL	0	NULL	cFos 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Light-dependent induction of cFos during subjective day and night in PACAP-containing ganglion cells of the retinohypothalamic tract .
	manualset3
113163	3	402308	13	NULL	NULL	0	NULL	day	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Light-dependent induction of cFos during subjective day and night in PACAP-containing ganglion cells of the retinohypothalamic tract .
	manualset3
113164	4	402308	13	NULL	NULL	0	NULL	night	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Light-dependent induction of cFos during subjective day and night in PACAP-containing ganglion cells of the retinohypothalamic tract .
	manualset3
113165	5	402308	13	NULL	NULL	0	NULL	PACAP-containing ganglion cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Light-dependent induction of cFos during subjective day and night in PACAP-containing ganglion cells of the retinohypothalamic tract .
	manualset3
113166	6	402308	13	NULL	NULL	0	NULL	retinohypothalamic tract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Light-dependent induction of cFos during subjective day and night in PACAP-containing ganglion cells of the retinohypothalamic tract .
	manualset3
113167	1	402309	13	NULL	NULL	0	NULL	Light -induced inactivation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Light - and DTT-induced inactivation are shown to be due to a Km shift with respect to glucose-6-phosphate ( G6P ) from 1 to 35 and 43 mM , respectively , and with respect to NADP from 10 to 50 microM without any significant change of the Vmax .
	manualset3
113168	2	402309	13	NULL	NULL	0	NULL	DTT-induced inactivation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Light - and DTT-induced inactivation are shown to be due to a Km shift with respect to glucose-6-phosphate ( G6P ) from 1 to 35 and 43 mM , respectively , and with respect to NADP from 10 to 50 microM without any significant change of the Vmax .
	manualset3
113169	3	402309	13	NULL	NULL	0	NULL	Km shift	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Light - and DTT-induced inactivation are shown to be due to a Km shift with respect to glucose-6-phosphate ( G6P ) from 1 to 35 and 43 mM , respectively , and with respect to NADP from 10 to 50 microM without any significant change of the Vmax .
	manualset3
113170	4	402309	13	NULL	NULL	0	NULL	respect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Light - and DTT-induced inactivation are shown to be due to a Km shift with respect to glucose-6-phosphate ( G6P ) from 1 to 35 and 43 mM , respectively , and with respect to NADP from 10 to 50 microM without any significant change of the Vmax .
	manualset3
113171	5	402309	13	NULL	NULL	0	NULL	glucose-6-phosphate ( G6P ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Light - and DTT-induced inactivation are shown to be due to a Km shift with respect to glucose-6-phosphate ( G6P ) from 1 to 35 and 43 mM , respectively , and with respect to NADP from 10 to 50 microM without any significant change of the Vmax .
	manualset3
113172	6	402309	13	NULL	NULL	0	NULL	1 to 35 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Light - and DTT-induced inactivation are shown to be due to a Km shift with respect to glucose-6-phosphate ( G6P ) from 1 to 35 and 43 mM , respectively , and with respect to NADP from 10 to 50 microM without any significant change of the Vmax .
	manualset3
113173	7	402309	13	NULL	NULL	0	NULL	43 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Light - and DTT-induced inactivation are shown to be due to a Km shift with respect to glucose-6-phosphate ( G6P ) from 1 to 35 and 43 mM , respectively , and with respect to NADP from 10 to 50 microM without any significant change of the Vmax .
	manualset3
113174	8	402309	13	NULL	NULL	0	NULL	respect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Light - and DTT-induced inactivation are shown to be due to a Km shift with respect to glucose-6-phosphate ( G6P ) from 1 to 35 and 43 mM , respectively , and with respect to NADP from 10 to 50 microM without any significant change of the Vmax .
	manualset3
113175	9	402309	13	NULL	NULL	0	NULL	NADP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Light - and DTT-induced inactivation are shown to be due to a Km shift with respect to glucose-6-phosphate ( G6P ) from 1 to 35 and 43 mM , respectively , and with respect to NADP from 10 to 50 microM without any significant change of the Vmax .
	manualset3
113176	10	402309	13	NULL	NULL	0	NULL	10 to 50 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Light - and DTT-induced inactivation are shown to be due to a Km shift with respect to glucose-6-phosphate ( G6P ) from 1 to 35 and 43 mM , respectively , and with respect to NADP from 10 to 50 microM without any significant change of the Vmax .
	manualset3
113177	11	402309	13	NULL	NULL	0	NULL	change 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Light - and DTT-induced inactivation are shown to be due to a Km shift with respect to glucose-6-phosphate ( G6P ) from 1 to 35 and 43 mM , respectively , and with respect to NADP from 10 to 50 microM without any significant change of the Vmax .
	manualset3
113178	12	402309	13	NULL	NULL	0	NULL	Vmax	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Light - and DTT-induced inactivation are shown to be due to a Km shift with respect to glucose-6-phosphate ( G6P ) from 1 to 35 and 43 mM , respectively , and with respect to NADP from 10 to 50 microM without any significant change of the Vmax .
	manualset3
113179	1	402310	13	NULL	NULL	0	NULL	38-year-old woman 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A 38-year-old woman had been treated with intravenous hydrocortisone , rectal steroid , and central venous alimentation for 6 weeks under the diagnosis of UC .
	manualset3
113180	2	402310	13	NULL	NULL	0	NULL	intravenous hydrocortisone	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A 38-year-old woman had been treated with intravenous hydrocortisone , rectal steroid , and central venous alimentation for 6 weeks under the diagnosis of UC .
	manualset3
113181	3	402310	13	NULL	NULL	0	NULL	rectal steroid	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A 38-year-old woman had been treated with intravenous hydrocortisone , rectal steroid , and central venous alimentation for 6 weeks under the diagnosis of UC .
	manualset3
113182	4	402310	13	NULL	NULL	0	NULL	central venous alimentation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A 38-year-old woman had been treated with intravenous hydrocortisone , rectal steroid , and central venous alimentation for 6 weeks under the diagnosis of UC .
	manualset3
113183	5	402310	13	NULL	NULL	0	NULL	6 weeks 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A 38-year-old woman had been treated with intravenous hydrocortisone , rectal steroid , and central venous alimentation for 6 weeks under the diagnosis of UC .
	manualset3
113184	6	402310	13	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A 38-year-old woman had been treated with intravenous hydrocortisone , rectal steroid , and central venous alimentation for 6 weeks under the diagnosis of UC .
	manualset3
113185	7	402310	13	NULL	NULL	0	NULL	UC	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 38-year-old woman had been treated with intravenous hydrocortisone , rectal steroid , and central venous alimentation for 6 weeks under the diagnosis of UC .
	manualset3
113186	1	402311	13	NULL	NULL	0	NULL	Light scattering 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Light scattering , vapor pressure osmometry , conductivity and surface tension techniques have been used to examine aqueous solutions of several narcotic analgesics for evidence of association .
	manualset3
113187	2	402311	13	NULL	NULL	0	NULL	vapor pressure osmometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Light scattering , vapor pressure osmometry , conductivity and surface tension techniques have been used to examine aqueous solutions of several narcotic analgesics for evidence of association .
	manualset3
113188	3	402311	13	NULL	NULL	0	NULL	conductivity technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Light scattering , vapor pressure osmometry , conductivity and surface tension techniques have been used to examine aqueous solutions of several narcotic analgesics for evidence of association .
	manualset3
113189	4	402311	13	NULL	NULL	0	NULL	surface tension technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Light scattering , vapor pressure osmometry , conductivity and surface tension techniques have been used to examine aqueous solutions of several narcotic analgesics for evidence of association .
	manualset3
113190	5	402311	13	NULL	NULL	0	NULL	aqueous solutions 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Light scattering , vapor pressure osmometry , conductivity and surface tension techniques have been used to examine aqueous solutions of several narcotic analgesics for evidence of association .
	manualset3
113191	6	402311	13	NULL	NULL	0	NULL	narcotic analgesics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Light scattering , vapor pressure osmometry , conductivity and surface tension techniques have been used to examine aqueous solutions of several narcotic analgesics for evidence of association .
	manualset3
113192	7	402311	13	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Light scattering , vapor pressure osmometry , conductivity and surface tension techniques have been used to examine aqueous solutions of several narcotic analgesics for evidence of association .
	manualset3
113193	8	402311	13	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Light scattering , vapor pressure osmometry , conductivity and surface tension techniques have been used to examine aqueous solutions of several narcotic analgesics for evidence of association .
	manualset3
113194	1	402312	13	NULL	NULL	0	NULL	Light scattering	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Light scattering by donor lenses as a function of depth and wavelength .
	manualset3
113195	2	402312	13	NULL	NULL	0	NULL	donor lenses	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Light scattering by donor lenses as a function of depth and wavelength .
	manualset3
113196	3	402312	13	NULL	NULL	0	NULL	function 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Light scattering by donor lenses as a function of depth and wavelength .
	manualset3
113197	4	402312	13	NULL	NULL	0	NULL	depth	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Light scattering by donor lenses as a function of depth and wavelength .
	manualset3
113198	5	402312	13	NULL	NULL	0	NULL	wavelength	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Light scattering by donor lenses as a function of depth and wavelength .
	manualset3
113199	1	402313	13	NULL	NULL	0	NULL	Lignin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lignin was the most sensitive component to the degradation process and underwent severe photodegradation during the process of irradiation .
	manualset3
113200	2	402313	13	NULL	NULL	0	NULL	component	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lignin was the most sensitive component to the degradation process and underwent severe photodegradation during the process of irradiation .
	manualset3
113201	3	402313	13	NULL	NULL	0	NULL	degradation process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Lignin was the most sensitive component to the degradation process and underwent severe photodegradation during the process of irradiation .
	manualset3
113202	4	402313	13	NULL	NULL	0	NULL	photodegradation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Lignin was the most sensitive component to the degradation process and underwent severe photodegradation during the process of irradiation .
	manualset3
113203	5	402313	13	NULL	NULL	0	NULL	process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Lignin was the most sensitive component to the degradation process and underwent severe photodegradation during the process of irradiation .
	manualset3
113204	6	402313	13	NULL	NULL	0	NULL	irradiation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Lignin was the most sensitive component to the degradation process and underwent severe photodegradation during the process of irradiation .
	manualset3
113205	1	402314	13	NULL	NULL	0	NULL	Ligustrazine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ligustrazine decreased MDA levels and ameliorated the down-regulation of SOD activity .
	manualset3
113206	2	402314	13	NULL	NULL	0	NULL	MDA levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ligustrazine decreased MDA levels and ameliorated the down-regulation of SOD activity .
	manualset3
113207	3	402314	13	NULL	NULL	0	NULL	down-regulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ligustrazine decreased MDA levels and ameliorated the down-regulation of SOD activity .
	manualset3
113208	4	402314	13	NULL	NULL	0	NULL	SOD activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ligustrazine decreased MDA levels and ameliorated the down-regulation of SOD activity .
	manualset3
113209	1	402315	13	NULL	NULL	0	NULL	ADA reports	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Like ADA and WHO reports , this committee adopts a classification based on etiologies , and presents a two-dimensional figure with etiologies and the state of insulin deficiency on different axis .
	manualset3
113210	2	402315	13	NULL	NULL	0	NULL	WHO reports	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Like ADA and WHO reports , this committee adopts a classification based on etiologies , and presents a two-dimensional figure with etiologies and the state of insulin deficiency on different axis .
	manualset3
113211	3	402315	13	NULL	NULL	0	NULL	committee	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Like ADA and WHO reports , this committee adopts a classification based on etiologies , and presents a two-dimensional figure with etiologies and the state of insulin deficiency on different axis .
	manualset3
113212	4	402315	13	NULL	NULL	0	NULL	adopts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Like ADA and WHO reports , this committee adopts a classification based on etiologies , and presents a two-dimensional figure with etiologies and the state of insulin deficiency on different axis .
	manualset3
113213	5	402315	13	NULL	NULL	0	NULL	classification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Like ADA and WHO reports , this committee adopts a classification based on etiologies , and presents a two-dimensional figure with etiologies and the state of insulin deficiency on different axis .
	manualset3
113214	6	402315	13	NULL	NULL	0	NULL	etiologies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Like ADA and WHO reports , this committee adopts a classification based on etiologies , and presents a two-dimensional figure with etiologies and the state of insulin deficiency on different axis .
	manualset3
113215	7	402315	13	NULL	NULL	0	NULL	two-dimensional figure	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Like ADA and WHO reports , this committee adopts a classification based on etiologies , and presents a two-dimensional figure with etiologies and the state of insulin deficiency on different axis .
	manualset3
113216	8	402315	13	NULL	NULL	0	NULL	etiologies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Like ADA and WHO reports , this committee adopts a classification based on etiologies , and presents a two-dimensional figure with etiologies and the state of insulin deficiency on different axis .
	manualset3
113217	9	402315	13	NULL	NULL	0	NULL	state of insulin deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Like ADA and WHO reports , this committee adopts a classification based on etiologies , and presents a two-dimensional figure with etiologies and the state of insulin deficiency on different axis .
	manualset3
113218	10	402315	13	NULL	NULL	0	NULL	axis	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Like ADA and WHO reports , this committee adopts a classification based on etiologies , and presents a two-dimensional figure with etiologies and the state of insulin deficiency on different axis .
	manualset3
113219	1	402316	13	NULL	NULL	0	NULL	human influenza viruses 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Like human influenza viruses , EIV H3N8 caused a transcontinental pandemic followed by further outbreaks and epidemics , even in populations with high vaccination coverage .
	manualset3
113220	2	402316	13	NULL	NULL	0	NULL	EIV H3N8 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Like human influenza viruses , EIV H3N8 caused a transcontinental pandemic followed by further outbreaks and epidemics , even in populations with high vaccination coverage .
	manualset3
113221	3	402316	13	NULL	NULL	0	NULL	transcontinental pandemic 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Like human influenza viruses , EIV H3N8 caused a transcontinental pandemic followed by further outbreaks and epidemics , even in populations with high vaccination coverage .
	manualset3
113222	4	402316	13	NULL	NULL	0	NULL	outbreaks 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Like human influenza viruses , EIV H3N8 caused a transcontinental pandemic followed by further outbreaks and epidemics , even in populations with high vaccination coverage .
	manualset3
113223	5	402316	13	NULL	NULL	0	NULL	epidemics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Like human influenza viruses , EIV H3N8 caused a transcontinental pandemic followed by further outbreaks and epidemics , even in populations with high vaccination coverage .
	manualset3
113224	6	402316	13	NULL	NULL	0	NULL	populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Like human influenza viruses , EIV H3N8 caused a transcontinental pandemic followed by further outbreaks and epidemics , even in populations with high vaccination coverage .
	manualset3
113225	7	402316	13	NULL	NULL	0	NULL	vaccination coverage	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Like human influenza viruses , EIV H3N8 caused a transcontinental pandemic followed by further outbreaks and epidemics , even in populations with high vaccination coverage .
	manualset3
113226	1	402317	13	NULL	NULL	0	NULL	human pDCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Like human pDCs , CD11c ( + ) Gr-1 ( + ) cells stimulate T cell proliferation after activation with CpG and produce IFNalpha after stimulation with influenza virus .
	manualset3
113227	2	402317	13	NULL	NULL	0	NULL	CD11c ( + ) Gr-1 ( + ) cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Like human pDCs , CD11c ( + ) Gr-1 ( + ) cells stimulate T cell proliferation after activation with CpG and produce IFNalpha after stimulation with influenza virus .
	manualset3
113228	3	402317	13	NULL	NULL	0	NULL	T cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Like human pDCs , CD11c ( + ) Gr-1 ( + ) cells stimulate T cell proliferation after activation with CpG and produce IFNalpha after stimulation with influenza virus .
	manualset3
113229	4	402317	13	NULL	NULL	0	NULL	activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Like human pDCs , CD11c ( + ) Gr-1 ( + ) cells stimulate T cell proliferation after activation with CpG and produce IFNalpha after stimulation with influenza virus .
	manualset3
113230	5	402317	13	NULL	NULL	0	NULL	CpG	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Like human pDCs , CD11c ( + ) Gr-1 ( + ) cells stimulate T cell proliferation after activation with CpG and produce IFNalpha after stimulation with influenza virus .
	manualset3
113231	6	402317	13	NULL	NULL	0	NULL	IFNalpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Like human pDCs , CD11c ( + ) Gr-1 ( + ) cells stimulate T cell proliferation after activation with CpG and produce IFNalpha after stimulation with influenza virus .
	manualset3
113232	7	402317	13	NULL	NULL	0	NULL	stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Like human pDCs , CD11c ( + ) Gr-1 ( + ) cells stimulate T cell proliferation after activation with CpG and produce IFNalpha after stimulation with influenza virus .
	manualset3
113233	8	402317	13	NULL	NULL	0	NULL	influenza virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Like human pDCs , CD11c ( + ) Gr-1 ( + ) cells stimulate T cell proliferation after activation with CpG and produce IFNalpha after stimulation with influenza virus .
	manualset3
113234	1	402318	13	NULL	NULL	0	NULL	ricin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Like ricin , the intoxication process of ML-1 may involve the Golgi regions .
	manualset3
113235	2	402318	13	NULL	NULL	0	NULL	intoxication process	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Like ricin , the intoxication process of ML-1 may involve the Golgi regions .
	manualset3
113236	3	402318	13	NULL	NULL	NULL	NULL	ML-1 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Like ricin , the intoxication process of ML-1 may involve the Golgi regions .
	manualset3
113237	4	402318	13	NULL	NULL	0	NULL	Golgi regions	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Like ricin , the intoxication process of ML-1 may involve the Golgi regions .
	manualset3
113238	1	402319	13	NULL	NULL	0	NULL	sodium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Like sodium , potassium too was not influenced by income and parity .
	manualset3
113239	2	402319	13	NULL	NULL	0	NULL	potassium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Like sodium , potassium too was not influenced by income and parity .
	manualset3
113240	3	402319	13	NULL	NULL	0	NULL	income	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Like sodium , potassium too was not influenced by income and parity .
	manualset3
113241	4	402319	13	NULL	NULL	0	NULL	parity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Like sodium , potassium too was not influenced by income and parity .
	manualset3
113242	1	402320	13	NULL	NULL	0	NULL	39-year-old pregnant woman	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A 39-year-old pregnant woman with fever after a trip to Africa .
	manualset3
113243	2	402320	13	NULL	NULL	0	NULL	fever	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 39-year-old pregnant woman with fever after a trip to Africa .
	manualset3
113244	3	402320	13	NULL	NULL	0	NULL	trip	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A 39-year-old pregnant woman with fever after a trip to Africa .
	manualset3
113245	4	402320	13	NULL	NULL	0	NULL	Africa	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A 39-year-old pregnant woman with fever after a trip to Africa .
	manualset3
113246	1	402321	13	NULL	NULL	0	NULL	basophils	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Like the basophils in normal individuals , most of these metachromatic cells contained segmented nuclei and expressed Bsp-1 .
	manualset3
113247	2	402321	13	NULL	NULL	0	NULL	normal individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Like the basophils in normal individuals , most of these metachromatic cells contained segmented nuclei and expressed Bsp-1 .
	manualset3
113248	3	402321	13	NULL	NULL	0	NULL	metachromatic cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Like the basophils in normal individuals , most of these metachromatic cells contained segmented nuclei and expressed Bsp-1 .
	manualset3
113249	4	402321	13	NULL	NULL	0	NULL	nuclei 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Like the basophils in normal individuals , most of these metachromatic cells contained segmented nuclei and expressed Bsp-1 .
	manualset3
113250	5	402321	13	NULL	NULL	0	NULL	Bsp-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Like the basophils in normal individuals , most of these metachromatic cells contained segmented nuclei and expressed Bsp-1 .
	manualset3
113251	1	402322	13	NULL	NULL	0	NULL	ubiquitination	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Like ubiquitination , sumoylation is a multistep process involving maturation , activation , conjugation and deconjugation .
	manualset3
113252	2	402322	13	NULL	NULL	0	NULL	sumoylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Like ubiquitination , sumoylation is a multistep process involving maturation , activation , conjugation and deconjugation .
	manualset3
113253	3	402322	13	NULL	NULL	0	NULL	multistep process	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Like ubiquitination , sumoylation is a multistep process involving maturation , activation , conjugation and deconjugation .
	manualset3
113254	4	402322	13	NULL	NULL	0	NULL	maturation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Like ubiquitination , sumoylation is a multistep process involving maturation , activation , conjugation and deconjugation .
	manualset3
113255	5	402322	13	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Like ubiquitination , sumoylation is a multistep process involving maturation , activation , conjugation and deconjugation .
	manualset3
113256	6	402322	13	NULL	NULL	0	NULL	conjugation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Like ubiquitination , sumoylation is a multistep process involving maturation , activation , conjugation and deconjugation .
	manualset3
113257	7	402322	13	NULL	NULL	0	NULL	deconjugation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Like ubiquitination , sumoylation is a multistep process involving maturation , activation , conjugation and deconjugation .
	manualset3
113258	1	402323	13	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , cells cultured for one , two , and three days with conditioned media ( CM ) obtained from MDA-MB-435 cells treated with VES exhibit 10 % , 36 % , and 74 % apoptosis , respectively .
	manualset3
113259	2	402323	13	NULL	NULL	0	NULL	one day	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , cells cultured for one , two , and three days with conditioned media ( CM ) obtained from MDA-MB-435 cells treated with VES exhibit 10 % , 36 % , and 74 % apoptosis , respectively .
	manualset3
113260	3	402323	13	NULL	NULL	0	NULL	two days	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , cells cultured for one , two , and three days with conditioned media ( CM ) obtained from MDA-MB-435 cells treated with VES exhibit 10 % , 36 % , and 74 % apoptosis , respectively .
	manualset3
113261	4	402323	13	NULL	NULL	0	NULL	three days	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , cells cultured for one , two , and three days with conditioned media ( CM ) obtained from MDA-MB-435 cells treated with VES exhibit 10 % , 36 % , and 74 % apoptosis , respectively .
	manualset3
113262	5	402323	13	NULL	NULL	0	NULL	 conditioned media ( CM )	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , cells cultured for one , two , and three days with conditioned media ( CM ) obtained from MDA-MB-435 cells treated with VES exhibit 10 % , 36 % , and 74 % apoptosis , respectively .
	manualset3
113263	6	402323	13	NULL	NULL	0	NULL	MDA-MB-435 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , cells cultured for one , two , and three days with conditioned media ( CM ) obtained from MDA-MB-435 cells treated with VES exhibit 10 % , 36 % , and 74 % apoptosis , respectively .
	manualset3
113264	7	402323	13	NULL	NULL	0	NULL	VES	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , cells cultured for one , two , and three days with conditioned media ( CM ) obtained from MDA-MB-435 cells treated with VES exhibit 10 % , 36 % , and 74 % apoptosis , respectively .
	manualset3
113265	8	402323	13	NULL	NULL	0	NULL	10 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , cells cultured for one , two , and three days with conditioned media ( CM ) obtained from MDA-MB-435 cells treated with VES exhibit 10 % , 36 % , and 74 % apoptosis , respectively .
	manualset3
113266	9	402323	13	NULL	NULL	0	NULL	36 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , cells cultured for one , two , and three days with conditioned media ( CM ) obtained from MDA-MB-435 cells treated with VES exhibit 10 % , 36 % , and 74 % apoptosis , respectively .
	manualset3
113267	10	402323	13	NULL	NULL	0	NULL	74 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , cells cultured for one , two , and three days with conditioned media ( CM ) obtained from MDA-MB-435 cells treated with VES exhibit 10 % , 36 % , and 74 % apoptosis , respectively .
	manualset3
113268	11	402323	13	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , cells cultured for one , two , and three days with conditioned media ( CM ) obtained from MDA-MB-435 cells treated with VES exhibit 10 % , 36 % , and 74 % apoptosis , respectively .
	manualset3
113269	1	402324	13	NULL	NULL	0	NULL	focal lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , dreaming is obliterated by focal lesions along a specific ( probably dopaminergic ) forebrain pathway , and these lesions do not have any appreciable effects on REM frequency , duration , and density .
	manualset3
113270	2	402324	13	NULL	NULL	0	NULL	forebrain pathway 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , dreaming is obliterated by focal lesions along a specific ( probably dopaminergic ) forebrain pathway , and these lesions do not have any appreciable effects on REM frequency , duration , and density .
	manualset3
113271	3	402324	13	NULL	NULL	0	NULL	lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , dreaming is obliterated by focal lesions along a specific ( probably dopaminergic ) forebrain pathway , and these lesions do not have any appreciable effects on REM frequency , duration , and density .
	manualset3
113272	4	402324	13	NULL	NULL	0	NULL	appreciable effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , dreaming is obliterated by focal lesions along a specific ( probably dopaminergic ) forebrain pathway , and these lesions do not have any appreciable effects on REM frequency , duration , and density .
	manualset3
113273	5	402324	13	NULL	NULL	0	NULL	REM frequency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , dreaming is obliterated by focal lesions along a specific ( probably dopaminergic ) forebrain pathway , and these lesions do not have any appreciable effects on REM frequency , duration , and density .
	manualset3
113274	6	402324	13	NULL	NULL	0	NULL	duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , dreaming is obliterated by focal lesions along a specific ( probably dopaminergic ) forebrain pathway , and these lesions do not have any appreciable effects on REM frequency , duration , and density .
	manualset3
113275	7	402324	13	NULL	NULL	0	NULL	density	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , dreaming is obliterated by focal lesions along a specific ( probably dopaminergic ) forebrain pathway , and these lesions do not have any appreciable effects on REM frequency , duration , and density .
	manualset3
113276	1	402325	13	NULL	NULL	0	NULL	high ambient temperatures	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , high ambient temperatures and humidity alter the intricate balance of endocrine profiles , leading to lower intensity of estrous behavior , anestrus , embryonic death , and subsequent infertility .
	manualset3
113277	2	402325	13	NULL	NULL	0	NULL	humidity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , high ambient temperatures and humidity alter the intricate balance of endocrine profiles , leading to lower intensity of estrous behavior , anestrus , embryonic death , and subsequent infertility .
	manualset3
113278	3	402325	13	NULL	NULL	0	NULL	 intricate balance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , high ambient temperatures and humidity alter the intricate balance of endocrine profiles , leading to lower intensity of estrous behavior , anestrus , embryonic death , and subsequent infertility .
	manualset3
113279	4	402325	13	NULL	NULL	0	NULL	endocrine profiles	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , high ambient temperatures and humidity alter the intricate balance of endocrine profiles , leading to lower intensity of estrous behavior , anestrus , embryonic death , and subsequent infertility .
	manualset3
113280	5	402325	13	NULL	NULL	0	NULL	lower intensity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , high ambient temperatures and humidity alter the intricate balance of endocrine profiles , leading to lower intensity of estrous behavior , anestrus , embryonic death , and subsequent infertility .
	manualset3
113281	6	402325	13	NULL	NULL	0	NULL	estrous behavior	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , high ambient temperatures and humidity alter the intricate balance of endocrine profiles , leading to lower intensity of estrous behavior , anestrus , embryonic death , and subsequent infertility .
	manualset3
113282	7	402325	13	NULL	NULL	0	NULL	embryonic death 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , high ambient temperatures and humidity alter the intricate balance of endocrine profiles , leading to lower intensity of estrous behavior , anestrus , embryonic death , and subsequent infertility .
	manualset3
113283	8	402325	13	NULL	NULL	0	NULL	subsequent infertility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , high ambient temperatures and humidity alter the intricate balance of endocrine profiles , leading to lower intensity of estrous behavior , anestrus , embryonic death , and subsequent infertility .
	manualset3
113360	1	402326	13	NULL	NULL	0	NULL	incubation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , incubation of 2-deoxyecdysone ( 2dE ) produced exclusively ecdysone ( E ) and 20E , indicating a high 2-hydroxylase activity in both tissues , despite calli not producing phytoecdysteroids .
	manualset3
113361	2	402326	13	NULL	NULL	0	NULL	2-deoxyecdysone ( 2dE ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , incubation of 2-deoxyecdysone ( 2dE ) produced exclusively ecdysone ( E ) and 20E , indicating a high 2-hydroxylase activity in both tissues , despite calli not producing phytoecdysteroids .
	manualset3
113362	3	402326	13	NULL	NULL	0	NULL	ecdysone ( E )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , incubation of 2-deoxyecdysone ( 2dE ) produced exclusively ecdysone ( E ) and 20E , indicating a high 2-hydroxylase activity in both tissues , despite calli not producing phytoecdysteroids .
	manualset3
113363	4	402326	13	NULL	NULL	0	NULL	20E	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , incubation of 2-deoxyecdysone ( 2dE ) produced exclusively ecdysone ( E ) and 20E , indicating a high 2-hydroxylase activity in both tissues , despite calli not producing phytoecdysteroids .
	manualset3
113364	5	402326	13	NULL	NULL	0	NULL	2-hydroxylase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , incubation of 2-deoxyecdysone ( 2dE ) produced exclusively ecdysone ( E ) and 20E , indicating a high 2-hydroxylase activity in both tissues , despite calli not producing phytoecdysteroids .
	manualset3
113365	6	402326	13	NULL	NULL	0	NULL	tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , incubation of 2-deoxyecdysone ( 2dE ) produced exclusively ecdysone ( E ) and 20E , indicating a high 2-hydroxylase activity in both tissues , despite calli not producing phytoecdysteroids .
	manualset3
113366	7	402326	13	NULL	NULL	0	NULL	calli	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , incubation of 2-deoxyecdysone ( 2dE ) produced exclusively ecdysone ( E ) and 20E , indicating a high 2-hydroxylase activity in both tissues , despite calli not producing phytoecdysteroids .
	manualset3
113367	8	402326	13	NULL	NULL	0	NULL	phytoecdysteroids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , incubation of 2-deoxyecdysone ( 2dE ) produced exclusively ecdysone ( E ) and 20E , indicating a high 2-hydroxylase activity in both tissues , despite calli not producing phytoecdysteroids .
	manualset3
113368	1	402327	13	NULL	NULL	0	NULL	protection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , no protection against the loss of heme , cytochrome P-450 , or enzymatic activity is afforded by inclusion of 1 mM dithiothreitol during the incubation with parathion , although the amount of irreversibly bound sulfur , i.e. sulfur not dissociable by dithiothreitol , is significantly reduced .
	manualset3
113369	2	402327	13	NULL	NULL	NULL	NULL	loss of heme	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Likewise , no protection against the loss of heme , cytochrome P-450 , or enzymatic activity is afforded by inclusion of 1 mM dithiothreitol during the incubation with parathion , although the amount of irreversibly bound sulfur , i.e. sulfur not dissociable by dithiothreitol , is significantly reduced .
	manualset3
113370	3	402327	13	NULL	NULL	0	NULL	cytochrome P-450	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , no protection against the loss of heme , cytochrome P-450 , or enzymatic activity is afforded by inclusion of 1 mM dithiothreitol during the incubation with parathion , although the amount of irreversibly bound sulfur , i.e. sulfur not dissociable by dithiothreitol , is significantly reduced .
	manualset3
113371	4	402327	13	NULL	NULL	0	NULL	enzymatic activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , no protection against the loss of heme , cytochrome P-450 , or enzymatic activity is afforded by inclusion of 1 mM dithiothreitol during the incubation with parathion , although the amount of irreversibly bound sulfur , i.e. sulfur not dissociable by dithiothreitol , is significantly reduced .
	manualset3
113372	5	402327	13	NULL	NULL	0	NULL	inclusion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , no protection against the loss of heme , cytochrome P-450 , or enzymatic activity is afforded by inclusion of 1 mM dithiothreitol during the incubation with parathion , although the amount of irreversibly bound sulfur , i.e. sulfur not dissociable by dithiothreitol , is significantly reduced .
	manualset3
113373	6	402327	13	NULL	NULL	0	NULL	1 mM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , no protection against the loss of heme , cytochrome P-450 , or enzymatic activity is afforded by inclusion of 1 mM dithiothreitol during the incubation with parathion , although the amount of irreversibly bound sulfur , i.e. sulfur not dissociable by dithiothreitol , is significantly reduced .
	manualset3
113374	7	402327	13	NULL	NULL	0	NULL	dithiothreitol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , no protection against the loss of heme , cytochrome P-450 , or enzymatic activity is afforded by inclusion of 1 mM dithiothreitol during the incubation with parathion , although the amount of irreversibly bound sulfur , i.e. sulfur not dissociable by dithiothreitol , is significantly reduced .
	manualset3
113375	8	402327	13	NULL	NULL	0	NULL	incubation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , no protection against the loss of heme , cytochrome P-450 , or enzymatic activity is afforded by inclusion of 1 mM dithiothreitol during the incubation with parathion , although the amount of irreversibly bound sulfur , i.e. sulfur not dissociable by dithiothreitol , is significantly reduced .
	manualset3
113376	9	402327	13	NULL	NULL	0	NULL	parathion	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , no protection against the loss of heme , cytochrome P-450 , or enzymatic activity is afforded by inclusion of 1 mM dithiothreitol during the incubation with parathion , although the amount of irreversibly bound sulfur , i.e. sulfur not dissociable by dithiothreitol , is significantly reduced .
	manualset3
113377	10	402327	13	NULL	NULL	0	NULL	amount 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , no protection against the loss of heme , cytochrome P-450 , or enzymatic activity is afforded by inclusion of 1 mM dithiothreitol during the incubation with parathion , although the amount of irreversibly bound sulfur , i.e. sulfur not dissociable by dithiothreitol , is significantly reduced .
	manualset3
113378	11	402327	13	NULL	NULL	0	NULL	sulfur	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , no protection against the loss of heme , cytochrome P-450 , or enzymatic activity is afforded by inclusion of 1 mM dithiothreitol during the incubation with parathion , although the amount of irreversibly bound sulfur , i.e. sulfur not dissociable by dithiothreitol , is significantly reduced .
	manualset3
113379	12	402327	13	NULL	NULL	0	NULL	sulfur	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , no protection against the loss of heme , cytochrome P-450 , or enzymatic activity is afforded by inclusion of 1 mM dithiothreitol during the incubation with parathion , although the amount of irreversibly bound sulfur , i.e. sulfur not dissociable by dithiothreitol , is significantly reduced .
	manualset3
113380	13	402327	13	NULL	NULL	0	NULL	dithiothreitol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Likewise , no protection against the loss of heme , cytochrome P-450 , or enzymatic activity is afforded by inclusion of 1 mM dithiothreitol during the incubation with parathion , although the amount of irreversibly bound sulfur , i.e. sulfur not dissociable by dithiothreitol , is significantly reduced .
	manualset3
113381	1	402328	13	NULL	NULL	0	NULL	4 years boy	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A 4 years boy with fulminant hepatitis due to virus A , underwent a temporary auxiliary liver transplantation .
	manualset3
113382	2	402328	13	NULL	NULL	0	NULL	fulminant hepatitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 4 years boy with fulminant hepatitis due to virus A , underwent a temporary auxiliary liver transplantation .
	manualset3
113383	3	402328	13	NULL	NULL	0	NULL	virus A	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A 4 years boy with fulminant hepatitis due to virus A , underwent a temporary auxiliary liver transplantation .
	manualset3
113384	4	402328	13	NULL	NULL	0	NULL	auxiliary liver transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A 4 years boy with fulminant hepatitis due to virus A , underwent a temporary auxiliary liver transplantation .
	manualset3
113385	1	402329	13	NULL	NULL	0	NULL	Limitations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Limitations in home monitoring technology have precluded longitudinal studies of hemoglobin oxygen saturation during unperturbed sleep .
	manualset3
113386	2	402329	13	NULL	NULL	0	NULL	home monitoring technology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Limitations in home monitoring technology have precluded longitudinal studies of hemoglobin oxygen saturation during unperturbed sleep .
	manualset3
113387	3	402329	13	NULL	NULL	0	NULL	longitudinal studies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Limitations in home monitoring technology have precluded longitudinal studies of hemoglobin oxygen saturation during unperturbed sleep .
	manualset3
113388	4	402329	13	NULL	NULL	0	NULL	hemoglobin oxygen saturation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Limitations in home monitoring technology have precluded longitudinal studies of hemoglobin oxygen saturation during unperturbed sleep .
	manualset3
113389	5	402329	13	NULL	NULL	0	NULL	unperturbed sleep	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Limitations in home monitoring technology have precluded longitudinal studies of hemoglobin oxygen saturation during unperturbed sleep .
	manualset3
113390	1	402330	13	NULL	NULL	0	NULL	Limitations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Limitations on residents ' working hours at New York teaching hospitals : a status report .
	manualset3
113391	2	402330	13	NULL	NULL	0	NULL	residents ' 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Limitations on residents ' working hours at New York teaching hospitals : a status report .
	manualset3
113392	3	402330	13	NULL	NULL	0	NULL	hours	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Limitations on residents ' working hours at New York teaching hospitals : a status report .
	manualset3
113393	4	402330	13	NULL	NULL	0	NULL	New York	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Limitations on residents ' working hours at New York teaching hospitals : a status report .
	manualset3
113394	5	402330	13	NULL	NULL	0	NULL	teaching hospitals	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Limitations on residents ' working hours at New York teaching hospitals : a status report .
	manualset3
113395	6	402330	13	NULL	NULL	0	NULL	status report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Limitations on residents ' working hours at New York teaching hospitals : a status report .
	manualset3
113396	1	402331	13	NULL	NULL	0	NULL	Limitations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Limitations on where persons would be allowed to smoke was seen as a viable government policy by the respondents .
	manualset3
113397	2	402331	13	NULL	NULL	0	NULL	persons	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Limitations on where persons would be allowed to smoke was seen as a viable government policy by the respondents .
	manualset3
113398	3	402331	13	NULL	NULL	0	NULL	government policy	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Limitations on where persons would be allowed to smoke was seen as a viable government policy by the respondents .
	manualset3
113399	4	402331	13	NULL	NULL	0	NULL	respondents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Limitations on where persons would be allowed to smoke was seen as a viable government policy by the respondents .
	manualset3
113400	1	402332	13	NULL	NULL	0	NULL	Limited proteolysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Limited proteolysis of myelin basic protein in a system mimetic of the myelin interlamellar aqueous space .
	manualset3
113401	2	402332	13	NULL	NULL	0	NULL	myelin basic protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Limited proteolysis of myelin basic protein in a system mimetic of the myelin interlamellar aqueous space .
	manualset3
113402	3	402332	13	NULL	NULL	0	NULL	system	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Limited proteolysis of myelin basic protein in a system mimetic of the myelin interlamellar aqueous space .
	manualset3
113403	4	402332	13	NULL	NULL	0	NULL	myelin interlamellar aqueous space 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Limited proteolysis of myelin basic protein in a system mimetic of the myelin interlamellar aqueous space .
	manualset3
113404	1	402333	13	NULL	NULL	0	NULL	Limited studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Limited studies and observations dating back to 60 years ago pointed out the importance of the Golden Horn as a fishery .
	manualset3
113405	2	402333	13	NULL	NULL	0	NULL	observations 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Limited studies and observations dating back to 60 years ago pointed out the importance of the Golden Horn as a fishery .
	manualset3
113406	3	402333	13	NULL	NULL	0	NULL	60 years ago	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Limited studies and observations dating back to 60 years ago pointed out the importance of the Golden Horn as a fishery .
	manualset3
113407	4	402333	13	NULL	NULL	0	NULL	importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Limited studies and observations dating back to 60 years ago pointed out the importance of the Golden Horn as a fishery .
	manualset3
113408	5	402333	13	NULL	NULL	0	NULL	Golden Horn	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Limited studies and observations dating back to 60 years ago pointed out the importance of the Golden Horn as a fishery .
	manualset3
113409	6	402333	13	NULL	NULL	0	NULL	fishery	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Limited studies and observations dating back to 60 years ago pointed out the importance of the Golden Horn as a fishery .
	manualset3
113410	1	402334	13	NULL	NULL	0	NULL	Linchpin synthons	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Linchpin synthons : metalation of aryl bromides bearing a potassium trifluoroborate moiety .
	manualset3
113411	2	402334	13	NULL	NULL	0	NULL	metalation of aryl bromides	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Linchpin synthons : metalation of aryl bromides bearing a potassium trifluoroborate moiety .
	manualset3
113412	3	402334	13	NULL	NULL	0	NULL	potassium trifluoroborate moiety 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Linchpin synthons : metalation of aryl bromides bearing a potassium trifluoroborate moiety .
	manualset3
113413	1	402335	13	NULL	NULL	0	NULL	Linear calibration curves 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Linear calibration curves were obtained over the concentration range of 0.20 to 40 g mL ( -1 ) for BHA , and 0.80 to 50 g mL ( -1 ) for PG , using NBD-Cl reagent .
	manualset3
113414	2	402335	13	NULL	NULL	NULL	NULL	concentration range 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Linear calibration curves were obtained over the concentration range of 0.20 to 40 g mL ( -1 ) for BHA , and 0.80 to 50 g mL ( -1 ) for PG , using NBD-Cl reagent .
	manualset3
113415	3	402335	13	NULL	NULL	0	NULL	 BHA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Linear calibration curves were obtained over the concentration range of 0.20 to 40 g mL ( -1 ) for BHA , and 0.80 to 50 g mL ( -1 ) for PG , using NBD-Cl reagent .
	manualset3
113416	4	402335	13	NULL	NULL	0	NULL	0.20 to 40 g mL ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Linear calibration curves were obtained over the concentration range of 0.20 to 40 g mL ( -1 ) for BHA , and 0.80 to 50 g mL ( -1 ) for PG , using NBD-Cl reagent .
	manualset3
113417	5	402335	13	NULL	NULL	0	NULL	0.80 to 50 g mL ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Linear calibration curves were obtained over the concentration range of 0.20 to 40 g mL ( -1 ) for BHA , and 0.80 to 50 g mL ( -1 ) for PG , using NBD-Cl reagent .
	manualset3
113418	6	402335	13	NULL	NULL	0	NULL	PG	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Linear calibration curves were obtained over the concentration range of 0.20 to 40 g mL ( -1 ) for BHA , and 0.80 to 50 g mL ( -1 ) for PG , using NBD-Cl reagent .
	manualset3
113419	7	402335	13	NULL	NULL	0	NULL	NBD-Cl reagent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Linear calibration curves were obtained over the concentration range of 0.20 to 40 g mL ( -1 ) for BHA , and 0.80 to 50 g mL ( -1 ) for PG , using NBD-Cl reagent .
	manualset3
113420	1	402336	13	NULL	NULL	0	NULL	41-year-old male patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A 41-year-old male patient underwent transurethral resection for multiple bladder tumors in January , 1979 .
	manualset3
113421	2	402336	13	NULL	NULL	0	NULL	 transurethral resection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A 41-year-old male patient underwent transurethral resection for multiple bladder tumors in January , 1979 .
	manualset3
113422	3	402336	13	NULL	NULL	0	NULL	multiple bladder tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 41-year-old male patient underwent transurethral resection for multiple bladder tumors in January , 1979 .
	manualset3
113423	4	402336	13	NULL	NULL	0	NULL	January , 1979	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	A 41-year-old male patient underwent transurethral resection for multiple bladder tumors in January , 1979 .
	manualset3
113424	1	402337	13	NULL	NULL	0	NULL	Linkage	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Linkage and sequence mutation analyses of the ADOA candidate genes OPA1 , OPA3 , OPA4 , and OPA5 , including the genes WFS1 , GJB2 , and GJB6 associated with recessive inherited OA or dominant LFSNHL , were performed .
	manualset3
113425	2	402337	13	NULL	NULL	0	NULL	sequence mutation analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Linkage and sequence mutation analyses of the ADOA candidate genes OPA1 , OPA3 , OPA4 , and OPA5 , including the genes WFS1 , GJB2 , and GJB6 associated with recessive inherited OA or dominant LFSNHL , were performed .
	manualset3
113426	3	402337	13	NULL	NULL	0	NULL	ADOA candidate genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Linkage and sequence mutation analyses of the ADOA candidate genes OPA1 , OPA3 , OPA4 , and OPA5 , including the genes WFS1 , GJB2 , and GJB6 associated with recessive inherited OA or dominant LFSNHL , were performed .
	manualset3
113427	4	402337	13	NULL	NULL	0	NULL	OPA1 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Linkage and sequence mutation analyses of the ADOA candidate genes OPA1 , OPA3 , OPA4 , and OPA5 , including the genes WFS1 , GJB2 , and GJB6 associated with recessive inherited OA or dominant LFSNHL , were performed .
	manualset3
113428	5	402337	13	NULL	NULL	0	NULL	OPA3	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Linkage and sequence mutation analyses of the ADOA candidate genes OPA1 , OPA3 , OPA4 , and OPA5 , including the genes WFS1 , GJB2 , and GJB6 associated with recessive inherited OA or dominant LFSNHL , were performed .
	manualset3
113429	6	402337	13	NULL	NULL	0	NULL	OPA4	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Linkage and sequence mutation analyses of the ADOA candidate genes OPA1 , OPA3 , OPA4 , and OPA5 , including the genes WFS1 , GJB2 , and GJB6 associated with recessive inherited OA or dominant LFSNHL , were performed .
	manualset3
113430	7	402337	13	NULL	NULL	0	NULL	OPA5	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Linkage and sequence mutation analyses of the ADOA candidate genes OPA1 , OPA3 , OPA4 , and OPA5 , including the genes WFS1 , GJB2 , and GJB6 associated with recessive inherited OA or dominant LFSNHL , were performed .
	manualset3
113431	8	402337	13	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Linkage and sequence mutation analyses of the ADOA candidate genes OPA1 , OPA3 , OPA4 , and OPA5 , including the genes WFS1 , GJB2 , and GJB6 associated with recessive inherited OA or dominant LFSNHL , were performed .
	manualset3
113432	9	402337	13	NULL	NULL	0	NULL	WFS1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Linkage and sequence mutation analyses of the ADOA candidate genes OPA1 , OPA3 , OPA4 , and OPA5 , including the genes WFS1 , GJB2 , and GJB6 associated with recessive inherited OA or dominant LFSNHL , were performed .
	manualset3
113433	10	402337	13	NULL	NULL	0	NULL	GJB2	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Linkage and sequence mutation analyses of the ADOA candidate genes OPA1 , OPA3 , OPA4 , and OPA5 , including the genes WFS1 , GJB2 , and GJB6 associated with recessive inherited OA or dominant LFSNHL , were performed .
	manualset3
113434	11	402337	13	NULL	NULL	0	NULL	GJB6	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Linkage and sequence mutation analyses of the ADOA candidate genes OPA1 , OPA3 , OPA4 , and OPA5 , including the genes WFS1 , GJB2 , and GJB6 associated with recessive inherited OA or dominant LFSNHL , were performed .
	manualset3
113435	12	402337	13	NULL	NULL	NULL	NULL	recessive inherited OA	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Linkage and sequence mutation analyses of the ADOA candidate genes OPA1 , OPA3 , OPA4 , and OPA5 , including the genes WFS1 , GJB2 , and GJB6 associated with recessive inherited OA or dominant LFSNHL , were performed .
	manualset3
113436	13	402337	13	NULL	NULL	0	NULL	dominant LFSNHL	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Linkage and sequence mutation analyses of the ADOA candidate genes OPA1 , OPA3 , OPA4 , and OPA5 , including the genes WFS1 , GJB2 , and GJB6 associated with recessive inherited OA or dominant LFSNHL , were performed .
	manualset3
113437	1	402338	13	NULL	NULL	0	NULL	Linkage relationships 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Linkage relationships of genes coding for alpha2-macroglobulin , C3 and C4 in the zebrafish : implications for the evolution of the complement and Mhc systems .
	manualset3
113438	2	402338	13	NULL	NULL	0	NULL	genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Linkage relationships of genes coding for alpha2-macroglobulin , C3 and C4 in the zebrafish : implications for the evolution of the complement and Mhc systems .
	manualset3
113439	3	402338	13	NULL	NULL	0	NULL	alpha2-macroglobulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Linkage relationships of genes coding for alpha2-macroglobulin , C3 and C4 in the zebrafish : implications for the evolution of the complement and Mhc systems .
	manualset3
113440	4	402338	13	NULL	NULL	0	NULL	C3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Linkage relationships of genes coding for alpha2-macroglobulin , C3 and C4 in the zebrafish : implications for the evolution of the complement and Mhc systems .
	manualset3
113441	5	402338	13	NULL	NULL	0	NULL	C4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Linkage relationships of genes coding for alpha2-macroglobulin , C3 and C4 in the zebrafish : implications for the evolution of the complement and Mhc systems .
	manualset3
113442	6	402338	13	NULL	NULL	0	NULL	zebrafish	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Linkage relationships of genes coding for alpha2-macroglobulin , C3 and C4 in the zebrafish : implications for the evolution of the complement and Mhc systems .
	manualset3
113443	7	402338	13	NULL	NULL	0	NULL	implications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Linkage relationships of genes coding for alpha2-macroglobulin , C3 and C4 in the zebrafish : implications for the evolution of the complement and Mhc systems .
	manualset3
113444	8	402338	13	NULL	NULL	0	NULL	evolution 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Linkage relationships of genes coding for alpha2-macroglobulin , C3 and C4 in the zebrafish : implications for the evolution of the complement and Mhc systems .
	manualset3
113445	9	402338	13	NULL	NULL	0	NULL	complement system	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Linkage relationships of genes coding for alpha2-macroglobulin , C3 and C4 in the zebrafish : implications for the evolution of the complement and Mhc systems .
	manualset3
113446	10	402338	13	NULL	NULL	0	NULL	Mhc system	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Linkage relationships of genes coding for alpha2-macroglobulin , C3 and C4 in the zebrafish : implications for the evolution of the complement and Mhc systems .
	manualset3
113447	1	402339	13	NULL	NULL	0	NULL	Linkage studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Linkage studies in affected families have already localized genes for several important diseases , including cystic fibrosis .
	manualset3
113448	2	402339	13	NULL	NULL	0	NULL	families	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Linkage studies in affected families have already localized genes for several important diseases , including cystic fibrosis .
	manualset3
113449	3	402339	13	NULL	NULL	0	NULL	genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Linkage studies in affected families have already localized genes for several important diseases , including cystic fibrosis .
	manualset3
113450	4	402339	13	NULL	NULL	0	NULL	diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Linkage studies in affected families have already localized genes for several important diseases , including cystic fibrosis .
	manualset3
113451	5	402339	13	NULL	NULL	0	NULL	cystic fibrosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Linkage studies in affected families have already localized genes for several important diseases , including cystic fibrosis .
	manualset3
113452	1	402340	13	NULL	NULL	0	NULL	Linoleic acid ( LA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Linoleic acid ( LA ) and its hydroperoxide 13-L-hydroperoxylinoleic acid ( LOOH ) prepared with soybean lipoxygenase inhibited the response of GABARs in the presence of GABA at high concentrations .
	manualset3
113453	2	402340	13	NULL	NULL	0	NULL	 hydroperoxide 13-L-hydroperoxylinoleic acid ( LOOH )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Linoleic acid ( LA ) and its hydroperoxide 13-L-hydroperoxylinoleic acid ( LOOH ) prepared with soybean lipoxygenase inhibited the response of GABARs in the presence of GABA at high concentrations .
	manualset3
113454	3	402340	13	NULL	NULL	0	NULL	soybean lipoxygenase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Linoleic acid ( LA ) and its hydroperoxide 13-L-hydroperoxylinoleic acid ( LOOH ) prepared with soybean lipoxygenase inhibited the response of GABARs in the presence of GABA at high concentrations .
	manualset3
113455	4	402340	13	NULL	NULL	0	NULL	response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Linoleic acid ( LA ) and its hydroperoxide 13-L-hydroperoxylinoleic acid ( LOOH ) prepared with soybean lipoxygenase inhibited the response of GABARs in the presence of GABA at high concentrations .
	manualset3
113456	5	402340	13	NULL	NULL	0	NULL	GABARs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Linoleic acid ( LA ) and its hydroperoxide 13-L-hydroperoxylinoleic acid ( LOOH ) prepared with soybean lipoxygenase inhibited the response of GABARs in the presence of GABA at high concentrations .
	manualset3
113457	6	402340	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Linoleic acid ( LA ) and its hydroperoxide 13-L-hydroperoxylinoleic acid ( LOOH ) prepared with soybean lipoxygenase inhibited the response of GABARs in the presence of GABA at high concentrations .
	manualset3
113458	7	402340	13	NULL	NULL	0	NULL	GABA 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Linoleic acid ( LA ) and its hydroperoxide 13-L-hydroperoxylinoleic acid ( LOOH ) prepared with soybean lipoxygenase inhibited the response of GABARs in the presence of GABA at high concentrations .
	manualset3
113459	8	402340	13	NULL	NULL	0	NULL	concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Linoleic acid ( LA ) and its hydroperoxide 13-L-hydroperoxylinoleic acid ( LOOH ) prepared with soybean lipoxygenase inhibited the response of GABARs in the presence of GABA at high concentrations .
	manualset3
113460	1	402341	13	NULL	NULL	0	NULL	Lipid IVA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipid IVA inhibits synthesis and release of tumor necrosis factor induced by lipopolysaccharide in human whole blood ex vivo .
	manualset3
113461	2	402341	13	NULL	NULL	0	NULL	synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipid IVA inhibits synthesis and release of tumor necrosis factor induced by lipopolysaccharide in human whole blood ex vivo .
	manualset3
113462	3	402341	13	NULL	NULL	0	NULL	release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipid IVA inhibits synthesis and release of tumor necrosis factor induced by lipopolysaccharide in human whole blood ex vivo .
	manualset3
113463	4	402341	13	NULL	NULL	0	NULL	tumor necrosis factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipid IVA inhibits synthesis and release of tumor necrosis factor induced by lipopolysaccharide in human whole blood ex vivo .
	manualset3
113464	5	402341	13	NULL	NULL	0	NULL	lipopolysaccharide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipid IVA inhibits synthesis and release of tumor necrosis factor induced by lipopolysaccharide in human whole blood ex vivo .
	manualset3
117413	6	402341	13	NULL	NULL	0	NULL	human whole blood 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipid IVA inhibits synthesis and release of tumor necrosis factor induced by lipopolysaccharide in human whole blood ex vivo .
	manualset3
113465	1	402342	13	NULL	NULL	NULL	NULL	Lipid domains	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Lipid domains of the plasma membrane were originally described as a cell matrix insoluble in cold - nonionic detergents and enriched in glycosphingolipids .
	manualset3
113466	2	402342	13	NULL	NULL	0	NULL	plasma membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipid domains of the plasma membrane were originally described as a cell matrix insoluble in cold - nonionic detergents and enriched in glycosphingolipids .
	manualset3
113467	3	402342	13	NULL	NULL	0	NULL	cell matrix	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipid domains of the plasma membrane were originally described as a cell matrix insoluble in cold - nonionic detergents and enriched in glycosphingolipids .
	manualset3
113468	4	402342	13	NULL	NULL	0	NULL	cold - nonionic detergents 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipid domains of the plasma membrane were originally described as a cell matrix insoluble in cold - nonionic detergents and enriched in glycosphingolipids .
	manualset3
113469	5	402342	13	NULL	NULL	0	NULL	glycosphingolipids 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipid domains of the plasma membrane were originally described as a cell matrix insoluble in cold - nonionic detergents and enriched in glycosphingolipids .
	manualset3
113470	1	402343	13	NULL	NULL	0	NULL	Lipid intermediates 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipid intermediates involved in the transfer of N-acetylglucosamine to proteins in baker 's yeast ( Saccharomyces cerevisiae ) .
	manualset3
113471	2	402343	13	NULL	NULL	0	NULL	transfer	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipid intermediates involved in the transfer of N-acetylglucosamine to proteins in baker 's yeast ( Saccharomyces cerevisiae ) .
	manualset3
113472	3	402343	13	NULL	NULL	0	NULL	N-acetylglucosamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipid intermediates involved in the transfer of N-acetylglucosamine to proteins in baker 's yeast ( Saccharomyces cerevisiae ) .
	manualset3
113473	4	402343	13	NULL	NULL	0	NULL	proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipid intermediates involved in the transfer of N-acetylglucosamine to proteins in baker 's yeast ( Saccharomyces cerevisiae ) .
	manualset3
113474	5	402343	13	NULL	NULL	0	NULL	baker 's yeast ( Saccharomyces cerevisiae )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipid intermediates involved in the transfer of N-acetylglucosamine to proteins in baker 's yeast ( Saccharomyces cerevisiae ) .
	manualset3
113475	1	402344	13	NULL	NULL	0	NULL	41-year-old man 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A 41-year-old man with 16 radial keratotomy ( RK ) incisions in each eye reported a paradoxical diurnal variation in vision in both eyes with low Dk/L soft contact lenses .
	manualset3
113476	2	402344	13	NULL	NULL	0	NULL	16	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A 41-year-old man with 16 radial keratotomy ( RK ) incisions in each eye reported a paradoxical diurnal variation in vision in both eyes with low Dk/L soft contact lenses .
	manualset3
113477	3	402344	13	NULL	NULL	0	NULL	radial keratotomy ( RK ) incisions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A 41-year-old man with 16 radial keratotomy ( RK ) incisions in each eye reported a paradoxical diurnal variation in vision in both eyes with low Dk/L soft contact lenses .
	manualset3
113478	4	402344	13	NULL	NULL	0	NULL	eye	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A 41-year-old man with 16 radial keratotomy ( RK ) incisions in each eye reported a paradoxical diurnal variation in vision in both eyes with low Dk/L soft contact lenses .
	manualset3
113479	5	402344	13	NULL	NULL	0	NULL	paradoxical diurnal variation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 41-year-old man with 16 radial keratotomy ( RK ) incisions in each eye reported a paradoxical diurnal variation in vision in both eyes with low Dk/L soft contact lenses .
	manualset3
113480	6	402344	13	NULL	NULL	0	NULL	vision 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 41-year-old man with 16 radial keratotomy ( RK ) incisions in each eye reported a paradoxical diurnal variation in vision in both eyes with low Dk/L soft contact lenses .
	manualset3
113481	7	402344	13	NULL	NULL	0	NULL	eyes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A 41-year-old man with 16 radial keratotomy ( RK ) incisions in each eye reported a paradoxical diurnal variation in vision in both eyes with low Dk/L soft contact lenses .
	manualset3
113482	8	402344	13	NULL	NULL	0	NULL	low Dk/L soft contact lenses 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A 41-year-old man with 16 radial keratotomy ( RK ) incisions in each eye reported a paradoxical diurnal variation in vision in both eyes with low Dk/L soft contact lenses .
	manualset3
113483	1	402345	13	NULL	NULL	0	NULL	Lipid metabolism 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipid metabolism and occurrence of post-percutaneous transluminal coronary angioplasty restenosis : role of cholesteryl ester transfer protein and paraoxonase/arylesterase .
	manualset3
113484	2	402345	13	NULL	NULL	0	NULL	occurrence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipid metabolism and occurrence of post-percutaneous transluminal coronary angioplasty restenosis : role of cholesteryl ester transfer protein and paraoxonase/arylesterase .
	manualset3
113485	3	402345	13	NULL	NULL	0	NULL	post-percutaneous transluminal coronary angioplasty restenosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipid metabolism and occurrence of post-percutaneous transluminal coronary angioplasty restenosis : role of cholesteryl ester transfer protein and paraoxonase/arylesterase .
	manualset3
113486	4	402345	13	NULL	NULL	0	NULL	role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipid metabolism and occurrence of post-percutaneous transluminal coronary angioplasty restenosis : role of cholesteryl ester transfer protein and paraoxonase/arylesterase .
	manualset3
113487	5	402345	13	NULL	NULL	0	NULL	cholesteryl ester transfer protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipid metabolism and occurrence of post-percutaneous transluminal coronary angioplasty restenosis : role of cholesteryl ester transfer protein and paraoxonase/arylesterase .
	manualset3
113488	6	402345	13	NULL	NULL	0	NULL	paraoxonase/arylesterase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipid metabolism and occurrence of post-percutaneous transluminal coronary angioplasty restenosis : role of cholesteryl ester transfer protein and paraoxonase/arylesterase .
	manualset3
113489	1	402346	13	NULL	NULL	0	NULL	Lipid peroxidation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipid peroxidation is a nonparenchymal cell event with reperfusion after prolonged liver ischemia .
	manualset3
113490	2	402346	13	NULL	NULL	0	NULL	nonparenchymal cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipid peroxidation is a nonparenchymal cell event with reperfusion after prolonged liver ischemia .
	manualset3
113491	3	402346	13	NULL	NULL	0	NULL	event	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipid peroxidation is a nonparenchymal cell event with reperfusion after prolonged liver ischemia .
	manualset3
113492	4	402346	13	NULL	NULL	0	NULL	reperfusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipid peroxidation is a nonparenchymal cell event with reperfusion after prolonged liver ischemia .
	manualset3
113493	5	402346	13	NULL	NULL	0	NULL	liver ischemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipid peroxidation is a nonparenchymal cell event with reperfusion after prolonged liver ischemia .
	manualset3
113494	1	402347	13	NULL	NULL	0	NULL	Lipocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipocytes survive for prolonged periods on plain plastic , and collagen synthesis by these cells remains relatively constant for at least 28 days .
	manualset3
113495	2	402347	13	NULL	NULL	0	NULL	periods	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipocytes survive for prolonged periods on plain plastic , and collagen synthesis by these cells remains relatively constant for at least 28 days .
	manualset3
113496	3	402347	13	NULL	NULL	0	NULL	plain plastic	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipocytes survive for prolonged periods on plain plastic , and collagen synthesis by these cells remains relatively constant for at least 28 days .
	manualset3
113497	4	402347	13	NULL	NULL	0	NULL	collagen synthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipocytes survive for prolonged periods on plain plastic , and collagen synthesis by these cells remains relatively constant for at least 28 days .
	manualset3
113498	5	402347	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipocytes survive for prolonged periods on plain plastic , and collagen synthesis by these cells remains relatively constant for at least 28 days .
	manualset3
113499	6	402347	13	NULL	NULL	NULL	NULL	28 days	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Lipocytes survive for prolonged periods on plain plastic , and collagen synthesis by these cells remains relatively constant for at least 28 days .
	manualset3
113500	1	402348	13	NULL	NULL	0	NULL	Lipoic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipoic acid , while reducing oxidative stress , normalized PKC activity and restored D1R-G ( q/11 ) alpha-PLC signaling and the ability of SKF-38393 to inhibit Na-K-ATPase activity .
	manualset3
113501	2	402348	13	NULL	NULL	0	NULL	oxidative stress	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipoic acid , while reducing oxidative stress , normalized PKC activity and restored D1R-G ( q/11 ) alpha-PLC signaling and the ability of SKF-38393 to inhibit Na-K-ATPase activity .
	manualset3
113502	3	402348	13	NULL	NULL	0	NULL	PKC activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipoic acid , while reducing oxidative stress , normalized PKC activity and restored D1R-G ( q/11 ) alpha-PLC signaling and the ability of SKF-38393 to inhibit Na-K-ATPase activity .
	manualset3
113503	4	402348	13	NULL	NULL	0	NULL	D1R-G ( q/11 ) alpha-PLC signaling 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipoic acid , while reducing oxidative stress , normalized PKC activity and restored D1R-G ( q/11 ) alpha-PLC signaling and the ability of SKF-38393 to inhibit Na-K-ATPase activity .
	manualset3
113504	5	402348	13	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipoic acid , while reducing oxidative stress , normalized PKC activity and restored D1R-G ( q/11 ) alpha-PLC signaling and the ability of SKF-38393 to inhibit Na-K-ATPase activity .
	manualset3
113505	6	402348	13	NULL	NULL	0	NULL	SKF-38393 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipoic acid , while reducing oxidative stress , normalized PKC activity and restored D1R-G ( q/11 ) alpha-PLC signaling and the ability of SKF-38393 to inhibit Na-K-ATPase activity .
	manualset3
113506	7	402348	13	NULL	NULL	0	NULL	Na-K-ATPase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipoic acid , while reducing oxidative stress , normalized PKC activity and restored D1R-G ( q/11 ) alpha-PLC signaling and the ability of SKF-38393 to inhibit Na-K-ATPase activity .
	manualset3
113507	1	402349	13	NULL	NULL	0	NULL	Lipoproteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipoproteins bearing truncated forms of apoB are cleared more rapidly than apoB-100 particles .
	manualset3
113508	2	402349	13	NULL	NULL	0	NULL	truncated forms of apoB	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipoproteins bearing truncated forms of apoB are cleared more rapidly than apoB-100 particles .
	manualset3
113509	3	402349	13	NULL	NULL	0	NULL	apoB-100 particles	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipoproteins bearing truncated forms of apoB are cleared more rapidly than apoB-100 particles .
	manualset3
113510	1	402350	13	NULL	NULL	0	NULL	42-year-old patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A 42-year-old patient presented with headache and a bilateral papillar edema .
	manualset3
113511	2	402350	13	NULL	NULL	0	NULL	headache	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 42-year-old patient presented with headache and a bilateral papillar edema .
	manualset3
113512	3	402350	13	NULL	NULL	0	NULL	bilateral papillar edema	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 42-year-old patient presented with headache and a bilateral papillar edema .
	manualset3
113513	1	402351	13	NULL	NULL	0	NULL	Liposome-encapsulated hemoglobin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Liposome-encapsulated hemoglobin alleviates hearing loss after transient cochlear ischemia and reperfusion in the gerbil .
	manualset3
113514	2	402351	13	NULL	NULL	0	NULL	hearing loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liposome-encapsulated hemoglobin alleviates hearing loss after transient cochlear ischemia and reperfusion in the gerbil .
	manualset3
113515	3	402351	13	NULL	NULL	0	NULL	transient cochlear ischemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liposome-encapsulated hemoglobin alleviates hearing loss after transient cochlear ischemia and reperfusion in the gerbil .
	manualset3
113516	4	402351	13	NULL	NULL	0	NULL	reperfusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liposome-encapsulated hemoglobin alleviates hearing loss after transient cochlear ischemia and reperfusion in the gerbil .
	manualset3
113517	5	402351	13	NULL	NULL	0	NULL	gerbil 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Liposome-encapsulated hemoglobin alleviates hearing loss after transient cochlear ischemia and reperfusion in the gerbil .
	manualset3
113518	1	402352	13	NULL	NULL	0	NULL	Lipoxygenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipoxygenase possessing dual catalytic activities , i.e. dioxygenase and hydroperoxidase , was purified from the cytosols of term placentas from non-smoking women .
	manualset3
113519	2	402352	13	NULL	NULL	0	NULL	catalytic activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipoxygenase possessing dual catalytic activities , i.e. dioxygenase and hydroperoxidase , was purified from the cytosols of term placentas from non-smoking women .
	manualset3
113520	3	402352	13	NULL	NULL	0	NULL	dioxygenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipoxygenase possessing dual catalytic activities , i.e. dioxygenase and hydroperoxidase , was purified from the cytosols of term placentas from non-smoking women .
	manualset3
113521	4	402352	13	NULL	NULL	0	NULL	hydroperoxidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipoxygenase possessing dual catalytic activities , i.e. dioxygenase and hydroperoxidase , was purified from the cytosols of term placentas from non-smoking women .
	manualset3
113522	5	402352	13	NULL	NULL	0	NULL	cytosols 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipoxygenase possessing dual catalytic activities , i.e. dioxygenase and hydroperoxidase , was purified from the cytosols of term placentas from non-smoking women .
	manualset3
113523	6	402352	13	NULL	NULL	0	NULL	placentas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipoxygenase possessing dual catalytic activities , i.e. dioxygenase and hydroperoxidase , was purified from the cytosols of term placentas from non-smoking women .
	manualset3
113524	7	402352	13	NULL	NULL	0	NULL	non-smoking women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Lipoxygenase possessing dual catalytic activities , i.e. dioxygenase and hydroperoxidase , was purified from the cytosols of term placentas from non-smoking women .
	manualset3
113525	1	402353	13	NULL	NULL	0	NULL	Liquid-solid circulating fluidized bed ( LSCFB )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Liquid-solid circulating fluidized bed ( LSCFB ) is an integrated two-column ( downcomer and riser ) system which can accommodate two separate processes ( adsorption and desorption ) in the same unit with continuous circulation of the solid particles between the two columns .
	manualset3
113526	2	402353	13	NULL	NULL	0	NULL	integrated two-column ( downcomer and riser ) system	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Liquid-solid circulating fluidized bed ( LSCFB ) is an integrated two-column ( downcomer and riser ) system which can accommodate two separate processes ( adsorption and desorption ) in the same unit with continuous circulation of the solid particles between the two columns .
	manualset3
113527	3	402353	13	NULL	NULL	0	NULL	processes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Liquid-solid circulating fluidized bed ( LSCFB ) is an integrated two-column ( downcomer and riser ) system which can accommodate two separate processes ( adsorption and desorption ) in the same unit with continuous circulation of the solid particles between the two columns .
	manualset3
113528	4	402353	13	NULL	NULL	0	NULL	adsorption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Liquid-solid circulating fluidized bed ( LSCFB ) is an integrated two-column ( downcomer and riser ) system which can accommodate two separate processes ( adsorption and desorption ) in the same unit with continuous circulation of the solid particles between the two columns .
	manualset3
113529	5	402353	13	NULL	NULL	0	NULL	desorption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Liquid-solid circulating fluidized bed ( LSCFB ) is an integrated two-column ( downcomer and riser ) system which can accommodate two separate processes ( adsorption and desorption ) in the same unit with continuous circulation of the solid particles between the two columns .
	manualset3
113530	6	402353	13	NULL	NULL	0	NULL	unit 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Liquid-solid circulating fluidized bed ( LSCFB ) is an integrated two-column ( downcomer and riser ) system which can accommodate two separate processes ( adsorption and desorption ) in the same unit with continuous circulation of the solid particles between the two columns .
	manualset3
113531	7	402353	13	NULL	NULL	0	NULL	circulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Liquid-solid circulating fluidized bed ( LSCFB ) is an integrated two-column ( downcomer and riser ) system which can accommodate two separate processes ( adsorption and desorption ) in the same unit with continuous circulation of the solid particles between the two columns .
	manualset3
113532	8	402353	13	NULL	NULL	0	NULL	solid particles	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Liquid-solid circulating fluidized bed ( LSCFB ) is an integrated two-column ( downcomer and riser ) system which can accommodate two separate processes ( adsorption and desorption ) in the same unit with continuous circulation of the solid particles between the two columns .
	manualset3
113533	9	402353	13	NULL	NULL	0	NULL	two columns	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Liquid-solid circulating fluidized bed ( LSCFB ) is an integrated two-column ( downcomer and riser ) system which can accommodate two separate processes ( adsorption and desorption ) in the same unit with continuous circulation of the solid particles between the two columns .
	manualset3
113534	1	402354	13	NULL	NULL	0	NULL	Liquid chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Liquid chromatography/diode array detection/mass spectrometry analysis also revealed the presence of fumiquinazolines A to F in both A. fumigatus wild-type and pesL strains .
	manualset3
113535	2	402354	13	NULL	NULL	0	NULL	diode array detection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Liquid chromatography/diode array detection/mass spectrometry analysis also revealed the presence of fumiquinazolines A to F in both A. fumigatus wild-type and pesL strains .
	manualset3
113536	3	402354	13	NULL	NULL	0	NULL	mass spectrometry analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Liquid chromatography/diode array detection/mass spectrometry analysis also revealed the presence of fumiquinazolines A to F in both A. fumigatus wild-type and pesL strains .
	manualset3
113537	4	402354	13	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Liquid chromatography/diode array detection/mass spectrometry analysis also revealed the presence of fumiquinazolines A to F in both A. fumigatus wild-type and pesL strains .
	manualset3
113538	5	402354	13	NULL	NULL	0	NULL	fumiquinazolines A to F	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Liquid chromatography/diode array detection/mass spectrometry analysis also revealed the presence of fumiquinazolines A to F in both A. fumigatus wild-type and pesL strains .
	manualset3
113539	6	402354	13	NULL	NULL	0	NULL	A. fumigatus wild-type 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Liquid chromatography/diode array detection/mass spectrometry analysis also revealed the presence of fumiquinazolines A to F in both A. fumigatus wild-type and pesL strains .
	manualset3
113540	7	402354	13	NULL	NULL	0	NULL	pesL strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Liquid chromatography/diode array detection/mass spectrometry analysis also revealed the presence of fumiquinazolines A to F in both A. fumigatus wild-type and pesL strains .
	manualset3
113541	1	402355	13	NULL	NULL	NULL	NULL	Liquid cultures	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Liquid cultures with cellulose and solid state fermentation cultures on wheat straw of the white-rot fungi Pleurotus ostreatus and Trametes versicolor and the brown-rot fungus Piptoporus betulinus were assayed for the free and solid fraction-bound activity of lignocellulose-degrading enzymes .
	manualset3
113542	2	402355	13	NULL	NULL	0	NULL	cellulose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Liquid cultures with cellulose and solid state fermentation cultures on wheat straw of the white-rot fungi Pleurotus ostreatus and Trametes versicolor and the brown-rot fungus Piptoporus betulinus were assayed for the free and solid fraction-bound activity of lignocellulose-degrading enzymes .
	manualset3
113543	3	402355	13	NULL	NULL	0	NULL	solid state fermentation cultures	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Liquid cultures with cellulose and solid state fermentation cultures on wheat straw of the white-rot fungi Pleurotus ostreatus and Trametes versicolor and the brown-rot fungus Piptoporus betulinus were assayed for the free and solid fraction-bound activity of lignocellulose-degrading enzymes .
	manualset3
113544	4	402355	13	NULL	NULL	0	NULL	wheat straw	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Liquid cultures with cellulose and solid state fermentation cultures on wheat straw of the white-rot fungi Pleurotus ostreatus and Trametes versicolor and the brown-rot fungus Piptoporus betulinus were assayed for the free and solid fraction-bound activity of lignocellulose-degrading enzymes .
	manualset3
113545	5	402355	13	NULL	NULL	0	NULL	 white-rot fungi Pleurotus ostreatus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Liquid cultures with cellulose and solid state fermentation cultures on wheat straw of the white-rot fungi Pleurotus ostreatus and Trametes versicolor and the brown-rot fungus Piptoporus betulinus were assayed for the free and solid fraction-bound activity of lignocellulose-degrading enzymes .
	manualset3
113546	6	402355	13	NULL	NULL	0	NULL	Trametes versicolor	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Liquid cultures with cellulose and solid state fermentation cultures on wheat straw of the white-rot fungi Pleurotus ostreatus and Trametes versicolor and the brown-rot fungus Piptoporus betulinus were assayed for the free and solid fraction-bound activity of lignocellulose-degrading enzymes .
	manualset3
113547	7	402355	13	NULL	NULL	0	NULL	brown-rot fungus Piptoporus betulinus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Liquid cultures with cellulose and solid state fermentation cultures on wheat straw of the white-rot fungi Pleurotus ostreatus and Trametes versicolor and the brown-rot fungus Piptoporus betulinus were assayed for the free and solid fraction-bound activity of lignocellulose-degrading enzymes .
	manualset3
113548	8	402355	13	NULL	NULL	NULL	NULL	solid fraction-bound activity 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Liquid cultures with cellulose and solid state fermentation cultures on wheat straw of the white-rot fungi Pleurotus ostreatus and Trametes versicolor and the brown-rot fungus Piptoporus betulinus were assayed for the free and solid fraction-bound activity of lignocellulose-degrading enzymes .
	manualset3
113549	9	402355	13	NULL	NULL	0	NULL	lignocellulose-degrading enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Liquid cultures with cellulose and solid state fermentation cultures on wheat straw of the white-rot fungi Pleurotus ostreatus and Trametes versicolor and the brown-rot fungus Piptoporus betulinus were assayed for the free and solid fraction-bound activity of lignocellulose-degrading enzymes .
	manualset3
113612	1	402356	13	NULL	NULL	0	NULL	Literacy publications 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Literacy publications : American Annals of the Deaf 1996 to 2000 .
	manualset3
113613	2	402356	13	NULL	NULL	0	NULL	American Annals of the Deaf 	Journal												NULL		0	NULL	NULL	NULL	NULL	NULL	Literacy publications : American Annals of the Deaf 1996 to 2000 .
	manualset3
113614	3	402356	13	NULL	NULL	0	NULL	1996 to 2000	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Literacy publications : American Annals of the Deaf 1996 to 2000 .
	manualset3
113615	1	402357	13	NULL	NULL	0	NULL	Literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Literature examining the issue of violence against women and its various theories was reviewed .
	manualset3
113616	2	402357	13	NULL	NULL	0	NULL	issue	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Literature examining the issue of violence against women and its various theories was reviewed .
	manualset3
113617	3	402357	13	NULL	NULL	0	NULL	violence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Literature examining the issue of violence against women and its various theories was reviewed .
	manualset3
113618	4	402357	13	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Literature examining the issue of violence against women and its various theories was reviewed .
	manualset3
113619	5	402357	13	NULL	NULL	0	NULL	various theories	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Literature examining the issue of violence against women and its various theories was reviewed .
	manualset3
113620	1	402358	13	NULL	NULL	0	NULL	Lithium ( Li )	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Lithium ( Li ) actively antagonises the inhibiting action of vinca alkaloids on human leukocyte chemotaxis ; it proved to be related to the activation of microtubular system , possibly mediated by its inhibiting effect on cyclic AMP .
	manualset3
113621	2	402358	13	NULL	NULL	0	NULL	action	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Lithium ( Li ) actively antagonises the inhibiting action of vinca alkaloids on human leukocyte chemotaxis ; it proved to be related to the activation of microtubular system , possibly mediated by its inhibiting effect on cyclic AMP .
	manualset3
113622	3	402358	13	NULL	NULL	0	NULL	vinca alkaloids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lithium ( Li ) actively antagonises the inhibiting action of vinca alkaloids on human leukocyte chemotaxis ; it proved to be related to the activation of microtubular system , possibly mediated by its inhibiting effect on cyclic AMP .
	manualset3
113623	4	402358	13	NULL	NULL	0	NULL	human leukocyte chemotaxis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lithium ( Li ) actively antagonises the inhibiting action of vinca alkaloids on human leukocyte chemotaxis ; it proved to be related to the activation of microtubular system , possibly mediated by its inhibiting effect on cyclic AMP .
	manualset3
113624	5	402358	13	NULL	NULL	0	NULL	activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lithium ( Li ) actively antagonises the inhibiting action of vinca alkaloids on human leukocyte chemotaxis ; it proved to be related to the activation of microtubular system , possibly mediated by its inhibiting effect on cyclic AMP .
	manualset3
113625	6	402358	13	NULL	NULL	0	NULL	microtubular system	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lithium ( Li ) actively antagonises the inhibiting action of vinca alkaloids on human leukocyte chemotaxis ; it proved to be related to the activation of microtubular system , possibly mediated by its inhibiting effect on cyclic AMP .
	manualset3
113626	7	402358	13	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Lithium ( Li ) actively antagonises the inhibiting action of vinca alkaloids on human leukocyte chemotaxis ; it proved to be related to the activation of microtubular system , possibly mediated by its inhibiting effect on cyclic AMP .
	manualset3
113627	8	402358	13	NULL	NULL	0	NULL	cyclic AMP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Lithium ( Li ) actively antagonises the inhibiting action of vinca alkaloids on human leukocyte chemotaxis ; it proved to be related to the activation of microtubular system , possibly mediated by its inhibiting effect on cyclic AMP .
	manualset3
113628	1	402359	13	NULL	NULL	0	NULL	Lithium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Lithium inhibits Ins-1 , 4 - P2 hydrolysis uncompetitively with a Ki of approximately 6 mM .
	manualset3
113629	2	402359	13	NULL	NULL	0	NULL	Ins-1 , 4 - P2 hydrolysis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Lithium inhibits Ins-1 , 4 - P2 hydrolysis uncompetitively with a Ki of approximately 6 mM .
	manualset3
113630	3	402359	13	NULL	NULL	0	NULL	Ki 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Lithium inhibits Ins-1 , 4 - P2 hydrolysis uncompetitively with a Ki of approximately 6 mM .
	manualset3
113631	4	402359	13	NULL	NULL	0	NULL	approximately 6 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Lithium inhibits Ins-1 , 4 - P2 hydrolysis uncompetitively with a Ki of approximately 6 mM .
	manualset3
113632	1	402360	13	NULL	NULL	0	NULL	Lithium intoxication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lithium intoxication : case report and review of treatment .
	manualset3
113633	2	402360	13	NULL	NULL	0	NULL	case report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Lithium intoxication : case report and review of treatment .
	manualset3
113634	3	402360	13	NULL	NULL	0	NULL	review of treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Lithium intoxication : case report and review of treatment .
	manualset3
113635	1	402361	13	NULL	NULL	0	NULL	Lithium 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Lithium is the standard treatment for acute mania , and its effectiveness is solidly supported by experimental evidence .
	manualset3
113636	2	402361	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Lithium is the standard treatment for acute mania , and its effectiveness is solidly supported by experimental evidence .
	manualset3
113637	3	402361	13	NULL	NULL	0	NULL	acute mania	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lithium is the standard treatment for acute mania , and its effectiveness is solidly supported by experimental evidence .
	manualset3
113638	4	402361	13	NULL	NULL	0	NULL	effectiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lithium is the standard treatment for acute mania , and its effectiveness is solidly supported by experimental evidence .
	manualset3
113639	5	402361	13	NULL	NULL	0	NULL	experimental evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Lithium is the standard treatment for acute mania , and its effectiveness is solidly supported by experimental evidence .
	manualset3
113640	1	402362	13	NULL	NULL	0	NULL	Little	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Little is known about involvement of DC in multiple sclerosis ( MS ) , where auto-aggressive T cells against myelin autoantigens are considered to contribute to inflammation and demyelination in the central nervous system .
	manualset3
113641	2	402362	13	NULL	NULL	0	NULL	involvement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Little is known about involvement of DC in multiple sclerosis ( MS ) , where auto-aggressive T cells against myelin autoantigens are considered to contribute to inflammation and demyelination in the central nervous system .
	manualset3
113642	3	402362	13	NULL	NULL	0	NULL	DC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Little is known about involvement of DC in multiple sclerosis ( MS ) , where auto-aggressive T cells against myelin autoantigens are considered to contribute to inflammation and demyelination in the central nervous system .
	manualset3
113643	4	402362	13	NULL	NULL	0	NULL	multiple sclerosis ( MS ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Little is known about involvement of DC in multiple sclerosis ( MS ) , where auto-aggressive T cells against myelin autoantigens are considered to contribute to inflammation and demyelination in the central nervous system .
	manualset3
113644	5	402362	13	NULL	NULL	0	NULL	auto-aggressive T cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Little is known about involvement of DC in multiple sclerosis ( MS ) , where auto-aggressive T cells against myelin autoantigens are considered to contribute to inflammation and demyelination in the central nervous system .
	manualset3
113645	6	402362	13	NULL	NULL	0	NULL	myelin autoantigens	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Little is known about involvement of DC in multiple sclerosis ( MS ) , where auto-aggressive T cells against myelin autoantigens are considered to contribute to inflammation and demyelination in the central nervous system .
	manualset3
113646	7	402362	13	NULL	NULL	0	NULL	inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Little is known about involvement of DC in multiple sclerosis ( MS ) , where auto-aggressive T cells against myelin autoantigens are considered to contribute to inflammation and demyelination in the central nervous system .
	manualset3
113647	8	402362	13	NULL	NULL	0	NULL	demyelination	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Little is known about involvement of DC in multiple sclerosis ( MS ) , where auto-aggressive T cells against myelin autoantigens are considered to contribute to inflammation and demyelination in the central nervous system .
	manualset3
113648	9	402362	13	NULL	NULL	0	NULL	central nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Little is known about involvement of DC in multiple sclerosis ( MS ) , where auto-aggressive T cells against myelin autoantigens are considered to contribute to inflammation and demyelination in the central nervous system .
	manualset3
113649	1	402363	13	NULL	NULL	0	NULL	Little	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Little is known about the factors leading to the identity and appearance of Hwp1 binding partners on cells lining the oral cavity .
	manualset3
113650	2	402363	13	NULL	NULL	0	NULL	factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Little is known about the factors leading to the identity and appearance of Hwp1 binding partners on cells lining the oral cavity .
	manualset3
113651	3	402363	13	NULL	NULL	0	NULL	identity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Little is known about the factors leading to the identity and appearance of Hwp1 binding partners on cells lining the oral cavity .
	manualset3
113652	4	402363	13	NULL	NULL	0	NULL	appearance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Little is known about the factors leading to the identity and appearance of Hwp1 binding partners on cells lining the oral cavity .
	manualset3
113653	5	402363	13	NULL	NULL	NULL	NULL	Hwp1 binding partners	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Little is known about the factors leading to the identity and appearance of Hwp1 binding partners on cells lining the oral cavity .
	manualset3
113654	6	402363	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Little is known about the factors leading to the identity and appearance of Hwp1 binding partners on cells lining the oral cavity .
	manualset3
113655	7	402363	13	NULL	NULL	0	NULL	oral cavity	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Little is known about the factors leading to the identity and appearance of Hwp1 binding partners on cells lining the oral cavity .
	manualset3
113656	1	402364	13	NULL	NULL	0	NULL	Little 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Little is known about the pathogenic mechanisms of IgA nephropathy , despite being the most prevalent form of glomerulonephritis in humans .
	manualset3
113657	2	402364	13	NULL	NULL	0	NULL	pathogenic mechanisms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Little is known about the pathogenic mechanisms of IgA nephropathy , despite being the most prevalent form of glomerulonephritis in humans .
	manualset3
113658	3	402364	13	NULL	NULL	0	NULL	IgA nephropathy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Little is known about the pathogenic mechanisms of IgA nephropathy , despite being the most prevalent form of glomerulonephritis in humans .
	manualset3
113659	4	402364	13	NULL	NULL	0	NULL	prevalent form of glomerulonephritis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Little is known about the pathogenic mechanisms of IgA nephropathy , despite being the most prevalent form of glomerulonephritis in humans .
	manualset3
113660	5	402364	13	NULL	NULL	0	NULL	humans	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Little is known about the pathogenic mechanisms of IgA nephropathy , despite being the most prevalent form of glomerulonephritis in humans .
	manualset3
113661	1	402365	13	NULL	NULL	0	NULL	Little research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Little research has been conducted on the characteristics of the literature of respiratory care .
	manualset3
113662	2	402365	13	NULL	NULL	0	NULL	characteristics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Little research has been conducted on the characteristics of the literature of respiratory care .
	manualset3
113663	3	402365	13	NULL	NULL	0	NULL	literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Little research has been conducted on the characteristics of the literature of respiratory care .
	manualset3
113664	4	402365	13	NULL	NULL	0	NULL	respiratory care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Little research has been conducted on the characteristics of the literature of respiratory care .
	manualset3
113665	1	402366	13	NULL	NULL	0	NULL	48-year-old woman 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A 48-year-old woman was admitted with neck tumors and cutaneous nodules .
	manualset3
113666	2	402366	13	NULL	NULL	0	NULL	neck tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 48-year-old woman was admitted with neck tumors and cutaneous nodules .
	manualset3
113667	3	402366	13	NULL	NULL	0	NULL	cutaneous nodules	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 48-year-old woman was admitted with neck tumors and cutaneous nodules .
	manualset3
113668	1	402367	13	NULL	NULL	0	NULL	Liu Wei Di Huang Tang ( LWDHT ) 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Liu Wei Di Huang Tang ( LWDHT ) , a Chinese prescription for strengthening the body resistance , restoring the normal functions of the body to consolidate the constitution , and nourishing and invigorating the kidney yin , has been used to prevent and treat severe hyperplasia of esophageal epithelium for many years .
	manualset3
113669	2	402367	13	NULL	NULL	0	NULL	Chinese prescription 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Liu Wei Di Huang Tang ( LWDHT ) , a Chinese prescription for strengthening the body resistance , restoring the normal functions of the body to consolidate the constitution , and nourishing and invigorating the kidney yin , has been used to prevent and treat severe hyperplasia of esophageal epithelium for many years .
	manualset3
113670	3	402367	13	NULL	NULL	0	NULL	body resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liu Wei Di Huang Tang ( LWDHT ) , a Chinese prescription for strengthening the body resistance , restoring the normal functions of the body to consolidate the constitution , and nourishing and invigorating the kidney yin , has been used to prevent and treat severe hyperplasia of esophageal epithelium for many years .
	manualset3
113671	4	402367	13	NULL	NULL	0	NULL	 normal functions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liu Wei Di Huang Tang ( LWDHT ) , a Chinese prescription for strengthening the body resistance , restoring the normal functions of the body to consolidate the constitution , and nourishing and invigorating the kidney yin , has been used to prevent and treat severe hyperplasia of esophageal epithelium for many years .
	manualset3
113672	5	402367	13	NULL	NULL	0	NULL	body 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Liu Wei Di Huang Tang ( LWDHT ) , a Chinese prescription for strengthening the body resistance , restoring the normal functions of the body to consolidate the constitution , and nourishing and invigorating the kidney yin , has been used to prevent and treat severe hyperplasia of esophageal epithelium for many years .
	manualset3
113673	6	402367	13	NULL	NULL	0	NULL	constitution	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liu Wei Di Huang Tang ( LWDHT ) , a Chinese prescription for strengthening the body resistance , restoring the normal functions of the body to consolidate the constitution , and nourishing and invigorating the kidney yin , has been used to prevent and treat severe hyperplasia of esophageal epithelium for many years .
	manualset3
113674	7	402367	13	NULL	NULL	0	NULL	 kidney 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Liu Wei Di Huang Tang ( LWDHT ) , a Chinese prescription for strengthening the body resistance , restoring the normal functions of the body to consolidate the constitution , and nourishing and invigorating the kidney yin , has been used to prevent and treat severe hyperplasia of esophageal epithelium for many years .
	manualset3
113675	8	402367	13	NULL	NULL	0	NULL	severe hyperplasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liu Wei Di Huang Tang ( LWDHT ) , a Chinese prescription for strengthening the body resistance , restoring the normal functions of the body to consolidate the constitution , and nourishing and invigorating the kidney yin , has been used to prevent and treat severe hyperplasia of esophageal epithelium for many years .
	manualset3
113676	9	402367	13	NULL	NULL	0	NULL	esophageal epithelium 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Liu Wei Di Huang Tang ( LWDHT ) , a Chinese prescription for strengthening the body resistance , restoring the normal functions of the body to consolidate the constitution , and nourishing and invigorating the kidney yin , has been used to prevent and treat severe hyperplasia of esophageal epithelium for many years .
	manualset3
113677	10	402367	13	NULL	NULL	0	NULL	years	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Liu Wei Di Huang Tang ( LWDHT ) , a Chinese prescription for strengthening the body resistance , restoring the normal functions of the body to consolidate the constitution , and nourishing and invigorating the kidney yin , has been used to prevent and treat severe hyperplasia of esophageal epithelium for many years .
	manualset3
113678	1	402368	13	NULL	NULL	0	NULL	Live animal real-time ultrasound scans	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Live animal real-time ultrasound scans and carcass measures were taken on 80 pigs comprising two sexes ( 42 barrows ; 38 gilts ) and two halothane genotypes ( 40 carriers and 40 negatives ) that were slaughtered between 108 and 148 kg live weight .
	manualset3
113679	2	402368	13	NULL	NULL	0	NULL	carcass measures 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Live animal real-time ultrasound scans and carcass measures were taken on 80 pigs comprising two sexes ( 42 barrows ; 38 gilts ) and two halothane genotypes ( 40 carriers and 40 negatives ) that were slaughtered between 108 and 148 kg live weight .
	manualset3
113680	3	402368	13	NULL	NULL	0	NULL	80 pigs	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Live animal real-time ultrasound scans and carcass measures were taken on 80 pigs comprising two sexes ( 42 barrows ; 38 gilts ) and two halothane genotypes ( 40 carriers and 40 negatives ) that were slaughtered between 108 and 148 kg live weight .
	manualset3
113681	4	402368	13	NULL	NULL	0	NULL	two sexes	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Live animal real-time ultrasound scans and carcass measures were taken on 80 pigs comprising two sexes ( 42 barrows ; 38 gilts ) and two halothane genotypes ( 40 carriers and 40 negatives ) that were slaughtered between 108 and 148 kg live weight .
	manualset3
113682	5	402368	13	NULL	NULL	0	NULL	42 barrows	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Live animal real-time ultrasound scans and carcass measures were taken on 80 pigs comprising two sexes ( 42 barrows ; 38 gilts ) and two halothane genotypes ( 40 carriers and 40 negatives ) that were slaughtered between 108 and 148 kg live weight .
	manualset3
113683	6	402368	13	NULL	NULL	0	NULL	38 gilts	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Live animal real-time ultrasound scans and carcass measures were taken on 80 pigs comprising two sexes ( 42 barrows ; 38 gilts ) and two halothane genotypes ( 40 carriers and 40 negatives ) that were slaughtered between 108 and 148 kg live weight .
	manualset3
113684	7	402368	13	NULL	NULL	NULL	NULL	two halothane genotypes	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Live animal real-time ultrasound scans and carcass measures were taken on 80 pigs comprising two sexes ( 42 barrows ; 38 gilts ) and two halothane genotypes ( 40 carriers and 40 negatives ) that were slaughtered between 108 and 148 kg live weight .
	manualset3
113685	8	402368	13	NULL	NULL	NULL	NULL	40 carriers 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Live animal real-time ultrasound scans and carcass measures were taken on 80 pigs comprising two sexes ( 42 barrows ; 38 gilts ) and two halothane genotypes ( 40 carriers and 40 negatives ) that were slaughtered between 108 and 148 kg live weight .
	manualset3
113686	9	402368	13	NULL	NULL	NULL	NULL	40 negatives	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Live animal real-time ultrasound scans and carcass measures were taken on 80 pigs comprising two sexes ( 42 barrows ; 38 gilts ) and two halothane genotypes ( 40 carriers and 40 negatives ) that were slaughtered between 108 and 148 kg live weight .
	manualset3
113687	10	402368	13	NULL	NULL	0	NULL	108 kg live weight	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Live animal real-time ultrasound scans and carcass measures were taken on 80 pigs comprising two sexes ( 42 barrows ; 38 gilts ) and two halothane genotypes ( 40 carriers and 40 negatives ) that were slaughtered between 108 and 148 kg live weight .
	manualset3
113688	11	402368	13	NULL	NULL	0	NULL	148 kg live weight 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Live animal real-time ultrasound scans and carcass measures were taken on 80 pigs comprising two sexes ( 42 barrows ; 38 gilts ) and two halothane genotypes ( 40 carriers and 40 negatives ) that were slaughtered between 108 and 148 kg live weight .
	manualset3
113689	1	402369	13	NULL	NULL	0	NULL	Liver phagocytic clearance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver and spleen phagocytic clearance of blood-borne microparticulate tissue debris and products of intravascular coagulation after trauma and surgical injury is an important mechanism to limit the deposition of debris in the pulmonary vascular bed .
	manualset3
113690	2	402369	13	NULL	NULL	0	NULL	spleen phagocytic clearance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver and spleen phagocytic clearance of blood-borne microparticulate tissue debris and products of intravascular coagulation after trauma and surgical injury is an important mechanism to limit the deposition of debris in the pulmonary vascular bed .
	manualset3
113691	3	402369	13	NULL	NULL	0	NULL	blood-borne microparticulate tissue debris	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver and spleen phagocytic clearance of blood-borne microparticulate tissue debris and products of intravascular coagulation after trauma and surgical injury is an important mechanism to limit the deposition of debris in the pulmonary vascular bed .
	manualset3
113692	4	402369	13	NULL	NULL	0	NULL	 products of intravascular coagulation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver and spleen phagocytic clearance of blood-borne microparticulate tissue debris and products of intravascular coagulation after trauma and surgical injury is an important mechanism to limit the deposition of debris in the pulmonary vascular bed .
	manualset3
113693	5	402369	13	NULL	NULL	0	NULL	trauma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver and spleen phagocytic clearance of blood-borne microparticulate tissue debris and products of intravascular coagulation after trauma and surgical injury is an important mechanism to limit the deposition of debris in the pulmonary vascular bed .
	manualset3
113694	6	402369	13	NULL	NULL	0	NULL	surgical injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver and spleen phagocytic clearance of blood-borne microparticulate tissue debris and products of intravascular coagulation after trauma and surgical injury is an important mechanism to limit the deposition of debris in the pulmonary vascular bed .
	manualset3
113695	7	402369	13	NULL	NULL	0	NULL	mechanism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver and spleen phagocytic clearance of blood-borne microparticulate tissue debris and products of intravascular coagulation after trauma and surgical injury is an important mechanism to limit the deposition of debris in the pulmonary vascular bed .
	manualset3
113696	8	402369	13	NULL	NULL	0	NULL	deposition of debris 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver and spleen phagocytic clearance of blood-borne microparticulate tissue debris and products of intravascular coagulation after trauma and surgical injury is an important mechanism to limit the deposition of debris in the pulmonary vascular bed .
	manualset3
113697	9	402369	13	NULL	NULL	0	NULL	pulmonary vascular bed	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver and spleen phagocytic clearance of blood-borne microparticulate tissue debris and products of intravascular coagulation after trauma and surgical injury is an important mechanism to limit the deposition of debris in the pulmonary vascular bed .
	manualset3
113698	1	402370	13	NULL	NULL	0	NULL	Liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver concentrations of 4-ene VPA and alpha-fluoro-4-ene VPA were 0.96 + / - 0.11 and 0.89 + / - 0.19 micromol/g of wet liver , respectively , at 1 hr after the dose .
	manualset3
113699	2	402370	13	NULL	NULL	0	NULL	concentrations 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver concentrations of 4-ene VPA and alpha-fluoro-4-ene VPA were 0.96 + / - 0.11 and 0.89 + / - 0.19 micromol/g of wet liver , respectively , at 1 hr after the dose .
	manualset3
113700	3	402370	13	NULL	NULL	0	NULL	4-ene VPA 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver concentrations of 4-ene VPA and alpha-fluoro-4-ene VPA were 0.96 + / - 0.11 and 0.89 + / - 0.19 micromol/g of wet liver , respectively , at 1 hr after the dose .
	manualset3
113701	4	402370	13	NULL	NULL	0	NULL	alpha-fluoro-4-ene VPA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver concentrations of 4-ene VPA and alpha-fluoro-4-ene VPA were 0.96 + / - 0.11 and 0.89 + / - 0.19 micromol/g of wet liver , respectively , at 1 hr after the dose .
	manualset3
113702	5	402370	13	NULL	NULL	0	NULL	0.96 + / - 0.11 micromol/g  	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver concentrations of 4-ene VPA and alpha-fluoro-4-ene VPA were 0.96 + / - 0.11 and 0.89 + / - 0.19 micromol/g of wet liver , respectively , at 1 hr after the dose .
	manualset3
113703	6	402370	13	NULL	NULL	0	NULL	0.89 + / - 0.19 micromol/g	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver concentrations of 4-ene VPA and alpha-fluoro-4-ene VPA were 0.96 + / - 0.11 and 0.89 + / - 0.19 micromol/g of wet liver , respectively , at 1 hr after the dose .
	manualset3
113704	7	402370	13	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver concentrations of 4-ene VPA and alpha-fluoro-4-ene VPA were 0.96 + / - 0.11 and 0.89 + / - 0.19 micromol/g of wet liver , respectively , at 1 hr after the dose .
	manualset3
113705	8	402370	13	NULL	NULL	0	NULL	1 hr	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver concentrations of 4-ene VPA and alpha-fluoro-4-ene VPA were 0.96 + / - 0.11 and 0.89 + / - 0.19 micromol/g of wet liver , respectively , at 1 hr after the dose .
	manualset3
113706	9	402370	13	NULL	NULL	0	NULL	dose	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver concentrations of 4-ene VPA and alpha-fluoro-4-ene VPA were 0.96 + / - 0.11 and 0.89 + / - 0.19 micromol/g of wet liver , respectively , at 1 hr after the dose .
	manualset3
113707	1	402371	13	NULL	NULL	0	NULL	Liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver involvement in eclampsia and preeclampsia is referred to as HELLP syndrome , and epigastric and right upper quadrant pain is often a symptom of severe preeclampsia and may be indicative of imminent convulsions .
	manualset3
113708	2	402371	13	NULL	NULL	0	NULL	eclampsia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver involvement in eclampsia and preeclampsia is referred to as HELLP syndrome , and epigastric and right upper quadrant pain is often a symptom of severe preeclampsia and may be indicative of imminent convulsions .
	manualset3
113709	3	402371	13	NULL	NULL	0	NULL	preeclampsia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver involvement in eclampsia and preeclampsia is referred to as HELLP syndrome , and epigastric and right upper quadrant pain is often a symptom of severe preeclampsia and may be indicative of imminent convulsions .
	manualset3
113710	4	402371	13	NULL	NULL	0	NULL	HELLP syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver involvement in eclampsia and preeclampsia is referred to as HELLP syndrome , and epigastric and right upper quadrant pain is often a symptom of severe preeclampsia and may be indicative of imminent convulsions .
	manualset3
113711	5	402371	13	NULL	NULL	0	NULL	epigastric pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver involvement in eclampsia and preeclampsia is referred to as HELLP syndrome , and epigastric and right upper quadrant pain is often a symptom of severe preeclampsia and may be indicative of imminent convulsions .
	manualset3
113712	6	402371	13	NULL	NULL	0	NULL	right upper quadrant pain 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver involvement in eclampsia and preeclampsia is referred to as HELLP syndrome , and epigastric and right upper quadrant pain is often a symptom of severe preeclampsia and may be indicative of imminent convulsions .
	manualset3
113713	7	402371	13	NULL	NULL	0	NULL	symptom	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver involvement in eclampsia and preeclampsia is referred to as HELLP syndrome , and epigastric and right upper quadrant pain is often a symptom of severe preeclampsia and may be indicative of imminent convulsions .
	manualset3
113714	8	402371	13	NULL	NULL	0	NULL	severe preeclampsia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver involvement in eclampsia and preeclampsia is referred to as HELLP syndrome , and epigastric and right upper quadrant pain is often a symptom of severe preeclampsia and may be indicative of imminent convulsions .
	manualset3
113715	9	402371	13	NULL	NULL	0	NULL	imminent convulsions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver involvement in eclampsia and preeclampsia is referred to as HELLP syndrome , and epigastric and right upper quadrant pain is often a symptom of severe preeclampsia and may be indicative of imminent convulsions .
	manualset3
113716	1	402372	13	NULL	NULL	0	NULL	Liver metastases 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver metastases are the most common site of distant failure after curative resection of colorectal cancer and a source of significant cancer-related morbidity and mortality .
	manualset3
113717	2	402372	13	NULL	NULL	0	NULL	common site	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver metastases are the most common site of distant failure after curative resection of colorectal cancer and a source of significant cancer-related morbidity and mortality .
	manualset3
113718	3	402372	13	NULL	NULL	0	NULL	distant failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver metastases are the most common site of distant failure after curative resection of colorectal cancer and a source of significant cancer-related morbidity and mortality .
	manualset3
113719	4	402372	13	NULL	NULL	0	NULL	curative resection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver metastases are the most common site of distant failure after curative resection of colorectal cancer and a source of significant cancer-related morbidity and mortality .
	manualset3
113720	5	402372	13	NULL	NULL	0	NULL	colorectal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver metastases are the most common site of distant failure after curative resection of colorectal cancer and a source of significant cancer-related morbidity and mortality .
	manualset3
113721	6	402372	13	NULL	NULL	0	NULL	source 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver metastases are the most common site of distant failure after curative resection of colorectal cancer and a source of significant cancer-related morbidity and mortality .
	manualset3
113722	7	402372	13	NULL	NULL	0	NULL	cancer-related morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver metastases are the most common site of distant failure after curative resection of colorectal cancer and a source of significant cancer-related morbidity and mortality .
	manualset3
113723	8	402372	13	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver metastases are the most common site of distant failure after curative resection of colorectal cancer and a source of significant cancer-related morbidity and mortality .
	manualset3
113724	1	402373	13	NULL	NULL	0	NULL	BRANCHES OF THESUPRACLAVICULAR PORTION OF THE BRACHIAL PLEXUS	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( BRANCHES OF THESUPRACLAVICULAR PORTION OF THE BRACHIAL PLEXUS ) .
	manualset3
113725	1	402374	13	NULL	NULL	0	NULL	 49-year-old man 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A 49-year-old man was admitted with exercise-induced chest pain .
	manualset3
113726	2	402374	13	NULL	NULL	0	NULL	exercise-induced chest pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 49-year-old man was admitted with exercise-induced chest pain .
	manualset3
113727	1	402375	13	NULL	NULL	0	NULL	Liver specimens	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver specimens were available for further histologic investigation in 11 of our own cases of GM .
	manualset3
113728	2	402375	13	NULL	NULL	0	NULL	histologic investigation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver specimens were available for further histologic investigation in 11 of our own cases of GM .
	manualset3
113729	3	402375	13	NULL	NULL	0	NULL	11	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver specimens were available for further histologic investigation in 11 of our own cases of GM .
	manualset3
113730	4	402375	13	NULL	NULL	0	NULL	cases of GM 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver specimens were available for further histologic investigation in 11 of our own cases of GM .
	manualset3
113731	1	402376	13	NULL	NULL	0	NULL	Liver transplantation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver transplantation is now an established technique to treat children with end-stage liver disease .
	manualset3
113732	2	402376	13	NULL	NULL	0	NULL	technique 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver transplantation is now an established technique to treat children with end-stage liver disease .
	manualset3
113733	3	402376	13	NULL	NULL	0	NULL	 children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver transplantation is now an established technique to treat children with end-stage liver disease .
	manualset3
113734	4	402376	13	NULL	NULL	0	NULL	end-stage liver disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver transplantation is now an established technique to treat children with end-stage liver disease .
	manualset3
113735	1	402377	13	NULL	NULL	0	NULL	Liver transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver transplantation may still be the most effective long-term treatment for localized HCC .
	manualset3
113736	2	402377	13	NULL	NULL	0	NULL	long-term treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver transplantation may still be the most effective long-term treatment for localized HCC .
	manualset3
113737	3	402377	13	NULL	NULL	0	NULL	localized HCC 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver transplantation may still be the most effective long-term treatment for localized HCC .
	manualset3
113738	1	402378	13	NULL	NULL	0	NULL	Living liver donors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Living liver donors : a coordinator 's perspective .
	manualset3
113739	2	402378	13	NULL	NULL	0	NULL	coordinator 's perspective 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Living liver donors : a coordinator 's perspective .
	manualset3
113740	1	402379	13	NULL	NULL	0	NULL	downregulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Load-mediated downregulation of myostatin mRNA is not sufficient to promote myofiber hypertrophy in humans : a cluster analysis .
	manualset3
113741	2	402379	13	NULL	NULL	0	NULL	myostatin mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Load-mediated downregulation of myostatin mRNA is not sufficient to promote myofiber hypertrophy in humans : a cluster analysis .
	manualset3
113742	3	402379	13	NULL	NULL	0	NULL	myofiber hypertrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Load-mediated downregulation of myostatin mRNA is not sufficient to promote myofiber hypertrophy in humans : a cluster analysis .
	manualset3
113743	4	402379	13	NULL	NULL	0	NULL	humans 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Load-mediated downregulation of myostatin mRNA is not sufficient to promote myofiber hypertrophy in humans : a cluster analysis .
	manualset3
113744	5	402379	13	NULL	NULL	0	NULL	cluster analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Load-mediated downregulation of myostatin mRNA is not sufficient to promote myofiber hypertrophy in humans : a cluster analysis .
	manualset3
113745	1	402380	13	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Loading cells with EGTA , even after peroxidation had already occurred , also prevented TBHP-induced cell death , indicating that buffering intracellular Ca2 + prevents cell killing .
	manualset3
113746	2	402380	13	NULL	NULL	0	NULL	EGTA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Loading cells with EGTA , even after peroxidation had already occurred , also prevented TBHP-induced cell death , indicating that buffering intracellular Ca2 + prevents cell killing .
	manualset3
113747	3	402380	13	NULL	NULL	0	NULL	peroxidation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Loading cells with EGTA , even after peroxidation had already occurred , also prevented TBHP-induced cell death , indicating that buffering intracellular Ca2 + prevents cell killing .
	manualset3
113748	4	402380	13	NULL	NULL	0	NULL	TBHP-induced cell death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Loading cells with EGTA , even after peroxidation had already occurred , also prevented TBHP-induced cell death , indicating that buffering intracellular Ca2 + prevents cell killing .
	manualset3
113749	5	402380	13	NULL	NULL	0	NULL	intracellular Ca2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Loading cells with EGTA , even after peroxidation had already occurred , also prevented TBHP-induced cell death , indicating that buffering intracellular Ca2 + prevents cell killing .
	manualset3
113750	6	402380	13	NULL	NULL	0	NULL	cell killing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Loading cells with EGTA , even after peroxidation had already occurred , also prevented TBHP-induced cell death , indicating that buffering intracellular Ca2 + prevents cell killing .
	manualset3
113751	1	402381	13	NULL	NULL	0	NULL	Lobulated mass	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lobulated mass on the back of the scalp .
	manualset3
113752	2	402381	13	NULL	NULL	0	NULL	back of the scalp	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Lobulated mass on the back of the scalp .
	manualset3
113753	1	402382	13	NULL	NULL	0	NULL	Local DNA features 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Local DNA features affect RNA-directed transcriptional gene silencing and DNA methylation .
	manualset3
113754	2	402382	13	NULL	NULL	0	NULL	RNA-directed transcriptional gene silencing	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Local DNA features affect RNA-directed transcriptional gene silencing and DNA methylation .
	manualset3
113755	3	402382	13	NULL	NULL	0	NULL	DNA methylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Local DNA features affect RNA-directed transcriptional gene silencing and DNA methylation .
	manualset3
113756	1	402383	13	NULL	NULL	0	NULL	Local changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Local changes in the distribution of metallothionein indicate interaction of cadmium and trace metal carrier proteins as a probable mechanism for impaired wound healing .
	manualset3
113757	2	402383	13	NULL	NULL	0	NULL	distribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Local changes in the distribution of metallothionein indicate interaction of cadmium and trace metal carrier proteins as a probable mechanism for impaired wound healing .
	manualset3
113758	3	402383	13	NULL	NULL	0	NULL	metallothionein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Local changes in the distribution of metallothionein indicate interaction of cadmium and trace metal carrier proteins as a probable mechanism for impaired wound healing .
	manualset3
113759	4	402383	13	NULL	NULL	0	NULL	interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Local changes in the distribution of metallothionein indicate interaction of cadmium and trace metal carrier proteins as a probable mechanism for impaired wound healing .
	manualset3
113760	5	402383	13	NULL	NULL	0	NULL	cadmium 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Local changes in the distribution of metallothionein indicate interaction of cadmium and trace metal carrier proteins as a probable mechanism for impaired wound healing .
	manualset3
113761	6	402383	13	NULL	NULL	0	NULL	trace metal carrier proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Local changes in the distribution of metallothionein indicate interaction of cadmium and trace metal carrier proteins as a probable mechanism for impaired wound healing .
	manualset3
113762	7	402383	13	NULL	NULL	0	NULL	mechanism 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Local changes in the distribution of metallothionein indicate interaction of cadmium and trace metal carrier proteins as a probable mechanism for impaired wound healing .
	manualset3
113763	8	402383	13	NULL	NULL	0	NULL	wound healing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Local changes in the distribution of metallothionein indicate interaction of cadmium and trace metal carrier proteins as a probable mechanism for impaired wound healing .
	manualset3
113764	1	402384	13	NULL	NULL	0	NULL	Local delivery	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Local delivery of basic fibroblast growth factor increases both angiogenesis and engraftment of hepatocytes in tissue-engineered polymer devices .
	manualset3
113765	2	402384	13	NULL	NULL	0	NULL	basic fibroblast growth factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Local delivery of basic fibroblast growth factor increases both angiogenesis and engraftment of hepatocytes in tissue-engineered polymer devices .
	manualset3
113766	3	402384	13	NULL	NULL	0	NULL	angiogenesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Local delivery of basic fibroblast growth factor increases both angiogenesis and engraftment of hepatocytes in tissue-engineered polymer devices .
	manualset3
113767	4	402384	13	NULL	NULL	0	NULL	engraftment	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Local delivery of basic fibroblast growth factor increases both angiogenesis and engraftment of hepatocytes in tissue-engineered polymer devices .
	manualset3
113768	5	402384	13	NULL	NULL	0	NULL	hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Local delivery of basic fibroblast growth factor increases both angiogenesis and engraftment of hepatocytes in tissue-engineered polymer devices .
	manualset3
113769	6	402384	13	NULL	NULL	0	NULL	tissue-engineered polymer devices	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Local delivery of basic fibroblast growth factor increases both angiogenesis and engraftment of hepatocytes in tissue-engineered polymer devices .
	manualset3
113770	1	402385	13	NULL	NULL	0	NULL	Local excision	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Local excision is curative , and there is no propensity to develop malignancy in these patients .
	manualset3
113771	2	402385	13	NULL	NULL	0	NULL	propensity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Local excision is curative , and there is no propensity to develop malignancy in these patients .
	manualset3
113772	3	402385	13	NULL	NULL	0	NULL	malignancy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Local excision is curative , and there is no propensity to develop malignancy in these patients .
	manualset3
113773	4	402385	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Local excision is curative , and there is no propensity to develop malignancy in these patients .
	manualset3
113826	1	402386	13	NULL	NULL	0	NULL	overexpression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Local overexpression of genes that promote lung defense or repair may be helpful in protecting the immature neonatal lung from injuries , but whether the vectors used to administer these genes affect physiological postnatal lung growth has not been investigated .
	manualset3
113827	2	402386	13	NULL	NULL	0	NULL	genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Local overexpression of genes that promote lung defense or repair may be helpful in protecting the immature neonatal lung from injuries , but whether the vectors used to administer these genes affect physiological postnatal lung growth has not been investigated .
	manualset3
113828	3	402386	13	NULL	NULL	0	NULL	lung defense	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Local overexpression of genes that promote lung defense or repair may be helpful in protecting the immature neonatal lung from injuries , but whether the vectors used to administer these genes affect physiological postnatal lung growth has not been investigated .
	manualset3
113829	4	402386	13	NULL	NULL	0	NULL	lung repair 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Local overexpression of genes that promote lung defense or repair may be helpful in protecting the immature neonatal lung from injuries , but whether the vectors used to administer these genes affect physiological postnatal lung growth has not been investigated .
	manualset3
113830	5	402386	13	NULL	NULL	0	NULL	neonatal lung	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Local overexpression of genes that promote lung defense or repair may be helpful in protecting the immature neonatal lung from injuries , but whether the vectors used to administer these genes affect physiological postnatal lung growth has not been investigated .
	manualset3
113831	6	402386	13	NULL	NULL	0	NULL	injuries 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Local overexpression of genes that promote lung defense or repair may be helpful in protecting the immature neonatal lung from injuries , but whether the vectors used to administer these genes affect physiological postnatal lung growth has not been investigated .
	manualset3
113832	7	402386	13	NULL	NULL	0	NULL	vectors	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Local overexpression of genes that promote lung defense or repair may be helpful in protecting the immature neonatal lung from injuries , but whether the vectors used to administer these genes affect physiological postnatal lung growth has not been investigated .
	manualset3
113833	8	402386	13	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Local overexpression of genes that promote lung defense or repair may be helpful in protecting the immature neonatal lung from injuries , but whether the vectors used to administer these genes affect physiological postnatal lung growth has not been investigated .
	manualset3
113834	9	402386	13	NULL	NULL	0	NULL	postnatal lung growth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Local overexpression of genes that promote lung defense or repair may be helpful in protecting the immature neonatal lung from injuries , but whether the vectors used to administer these genes affect physiological postnatal lung growth has not been investigated .
	manualset3
113835	1	402387	13	NULL	NULL	0	NULL	Local pressure application	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Local pressure application of Win 55212-3 ( the much less active enantiomer of WIN2 ) produced an insignificant decrease in SNpr firing rate .
	manualset3
113836	2	402387	13	NULL	NULL	0	NULL	Win 55212-3 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Local pressure application of Win 55212-3 ( the much less active enantiomer of WIN2 ) produced an insignificant decrease in SNpr firing rate .
	manualset3
113837	3	402387	13	NULL	NULL	0	NULL	enantiomer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Local pressure application of Win 55212-3 ( the much less active enantiomer of WIN2 ) produced an insignificant decrease in SNpr firing rate .
	manualset3
113838	4	402387	13	NULL	NULL	0	NULL	WIN2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Local pressure application of Win 55212-3 ( the much less active enantiomer of WIN2 ) produced an insignificant decrease in SNpr firing rate .
	manualset3
113839	5	402387	13	NULL	NULL	0	NULL	decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Local pressure application of Win 55212-3 ( the much less active enantiomer of WIN2 ) produced an insignificant decrease in SNpr firing rate .
	manualset3
113840	6	402387	13	NULL	NULL	0	NULL	SNpr firing rate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Local pressure application of Win 55212-3 ( the much less active enantiomer of WIN2 ) produced an insignificant decrease in SNpr firing rate .
	manualset3
113841	1	402388	13	NULL	NULL	0	NULL	Local routes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Local routes for immunotherapy ( IT ) such as oral ( OIT ) and sublingual ( SLIT ) have the primary aim of avoiding or minimizing the risk of adverse events and of improving the compliance of the patients with IT itself .
	manualset3
113842	2	402388	13	NULL	NULL	0	NULL	immunotherapy ( IT )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Local routes for immunotherapy ( IT ) such as oral ( OIT ) and sublingual ( SLIT ) have the primary aim of avoiding or minimizing the risk of adverse events and of improving the compliance of the patients with IT itself .
	manualset3
113843	3	402388	13	NULL	NULL	0	NULL	oral ( OIT ) 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Local routes for immunotherapy ( IT ) such as oral ( OIT ) and sublingual ( SLIT ) have the primary aim of avoiding or minimizing the risk of adverse events and of improving the compliance of the patients with IT itself .
	manualset3
113844	4	402388	13	NULL	NULL	0	NULL	sublingual ( SLIT )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Local routes for immunotherapy ( IT ) such as oral ( OIT ) and sublingual ( SLIT ) have the primary aim of avoiding or minimizing the risk of adverse events and of improving the compliance of the patients with IT itself .
	manualset3
113845	5	402388	13	NULL	NULL	0	NULL	aim	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Local routes for immunotherapy ( IT ) such as oral ( OIT ) and sublingual ( SLIT ) have the primary aim of avoiding or minimizing the risk of adverse events and of improving the compliance of the patients with IT itself .
	manualset3
113846	6	402388	13	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Local routes for immunotherapy ( IT ) such as oral ( OIT ) and sublingual ( SLIT ) have the primary aim of avoiding or minimizing the risk of adverse events and of improving the compliance of the patients with IT itself .
	manualset3
113847	7	402388	13	NULL	NULL	0	NULL	adverse events 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Local routes for immunotherapy ( IT ) such as oral ( OIT ) and sublingual ( SLIT ) have the primary aim of avoiding or minimizing the risk of adverse events and of improving the compliance of the patients with IT itself .
	manualset3
113848	8	402388	13	NULL	NULL	0	NULL	compliance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Local routes for immunotherapy ( IT ) such as oral ( OIT ) and sublingual ( SLIT ) have the primary aim of avoiding or minimizing the risk of adverse events and of improving the compliance of the patients with IT itself .
	manualset3
113849	9	402388	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Local routes for immunotherapy ( IT ) such as oral ( OIT ) and sublingual ( SLIT ) have the primary aim of avoiding or minimizing the risk of adverse events and of improving the compliance of the patients with IT itself .
	manualset3
113850	10	402388	13	NULL	NULL	0	NULL	IT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Local routes for immunotherapy ( IT ) such as oral ( OIT ) and sublingual ( SLIT ) have the primary aim of avoiding or minimizing the risk of adverse events and of improving the compliance of the patients with IT itself .
	manualset3
113851	1	402389	13	NULL	NULL	0	NULL	Local screening program 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Local screening program sponsors should be cognizant that the health care needs and limited resources of some target populations may be substantial .
	manualset3
113852	2	402389	13	NULL	NULL	0	NULL	sponsors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Local screening program sponsors should be cognizant that the health care needs and limited resources of some target populations may be substantial .
	manualset3
113853	3	402389	13	NULL	NULL	0	NULL	health care needs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Local screening program sponsors should be cognizant that the health care needs and limited resources of some target populations may be substantial .
	manualset3
113854	4	402389	13	NULL	NULL	0	NULL	resources	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Local screening program sponsors should be cognizant that the health care needs and limited resources of some target populations may be substantial .
	manualset3
113855	5	402389	13	NULL	NULL	0	NULL	target populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Local screening program sponsors should be cognizant that the health care needs and limited resources of some target populations may be substantial .
	manualset3
113856	1	402390	13	NULL	NULL	0	NULL	Localization 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Localization of a novel melanoma susceptibility locus to 1p22 .
	manualset3
113857	2	402390	13	NULL	NULL	0	NULL	novel melanoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Localization of a novel melanoma susceptibility locus to 1p22 .
	manualset3
113858	3	402390	13	NULL	NULL	NULL	NULL	susceptibility locus	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Localization of a novel melanoma susceptibility locus to 1p22 .
	manualset3
113860	4	402390	13	NULL	NULL	0	NULL	1p22	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Localization of a novel melanoma susceptibility locus to 1p22 .
	manualset3
113861	1	402391	13	NULL	NULL	0	NULL	58-year-old man	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A 58-year-old man presented with knee pain and swelling , following a previous injury .
	manualset3
113862	2	402391	13	NULL	NULL	0	NULL	knee pain 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 58-year-old man presented with knee pain and swelling , following a previous injury .
	manualset3
113863	3	402391	13	NULL	NULL	0	NULL	previous injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 58-year-old man presented with knee pain and swelling , following a previous injury .
	manualset3
113864	4	402391	13	NULL	NULL	0	NULL	swelling	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 58-year-old man presented with knee pain and swelling , following a previous injury .
	manualset3
113865	1	402392	13	NULL	NULL	0	NULL	Localization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Localization of aquaporin-2 , renal morphology and urine composition in the bottlenose dolphin and the Baird 's beaked whale .
	manualset3
113866	2	402392	13	NULL	NULL	0	NULL	aquaporin-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Localization of aquaporin-2 , renal morphology and urine composition in the bottlenose dolphin and the Baird 's beaked whale .
	manualset3
113867	3	402392	13	NULL	NULL	0	NULL	renal morphology 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Localization of aquaporin-2 , renal morphology and urine composition in the bottlenose dolphin and the Baird 's beaked whale .
	manualset3
113868	4	402392	13	NULL	NULL	0	NULL	urine composition 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Localization of aquaporin-2 , renal morphology and urine composition in the bottlenose dolphin and the Baird 's beaked whale .
	manualset3
113869	5	402392	13	NULL	NULL	0	NULL	bottlenose dolphin 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Localization of aquaporin-2 , renal morphology and urine composition in the bottlenose dolphin and the Baird 's beaked whale .
	manualset3
113870	6	402392	13	NULL	NULL	0	NULL	Baird 's beaked whale	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Localization of aquaporin-2 , renal morphology and urine composition in the bottlenose dolphin and the Baird 's beaked whale .
	manualset3
113871	1	402393	13	NULL	NULL	0	NULL	Localization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Localization of the major olive allergen at ultrastructural level showed the protein present mainly in the lumen of the endoplasmic reticulum vesicles or pockets scattered in the cytoplasm , and in the outer region of the pollen exine .
	manualset3
113872	2	402393	13	NULL	NULL	0	NULL	olive allergen	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Localization of the major olive allergen at ultrastructural level showed the protein present mainly in the lumen of the endoplasmic reticulum vesicles or pockets scattered in the cytoplasm , and in the outer region of the pollen exine .
	manualset3
113874	3	402393	13	NULL	NULL	0	NULL	ultrastructural level 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Localization of the major olive allergen at ultrastructural level showed the protein present mainly in the lumen of the endoplasmic reticulum vesicles or pockets scattered in the cytoplasm , and in the outer region of the pollen exine .
	manualset3
113875	4	402393	13	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Localization of the major olive allergen at ultrastructural level showed the protein present mainly in the lumen of the endoplasmic reticulum vesicles or pockets scattered in the cytoplasm , and in the outer region of the pollen exine .
	manualset3
113876	5	402393	13	NULL	NULL	0	NULL	lumen	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Localization of the major olive allergen at ultrastructural level showed the protein present mainly in the lumen of the endoplasmic reticulum vesicles or pockets scattered in the cytoplasm , and in the outer region of the pollen exine .
	manualset3
113877	6	402393	13	NULL	NULL	0	NULL	endoplasmic reticulum vesicles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Localization of the major olive allergen at ultrastructural level showed the protein present mainly in the lumen of the endoplasmic reticulum vesicles or pockets scattered in the cytoplasm , and in the outer region of the pollen exine .
	manualset3
113878	7	402393	13	NULL	NULL	0	NULL	pockets	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Localization of the major olive allergen at ultrastructural level showed the protein present mainly in the lumen of the endoplasmic reticulum vesicles or pockets scattered in the cytoplasm , and in the outer region of the pollen exine .
	manualset3
113879	8	402393	13	NULL	NULL	0	NULL	cytoplasm	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Localization of the major olive allergen at ultrastructural level showed the protein present mainly in the lumen of the endoplasmic reticulum vesicles or pockets scattered in the cytoplasm , and in the outer region of the pollen exine .
	manualset3
113880	9	402393	13	NULL	NULL	0	NULL	outer region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Localization of the major olive allergen at ultrastructural level showed the protein present mainly in the lumen of the endoplasmic reticulum vesicles or pockets scattered in the cytoplasm , and in the outer region of the pollen exine .
	manualset3
113881	10	402393	13	NULL	NULL	0	NULL	pollen exine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Localization of the major olive allergen at ultrastructural level showed the protein present mainly in the lumen of the endoplasmic reticulum vesicles or pockets scattered in the cytoplasm , and in the outer region of the pollen exine .
	manualset3
113906	1	402394	13	NULL	NULL	0	NULL	Localization studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Localization studies with the labeled polypeptide in the T7-RNA polymerase system also suggest that ExuT is a membrane protein .
	manualset3
113907	2	402394	13	NULL	NULL	0	NULL	polypeptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Localization studies with the labeled polypeptide in the T7-RNA polymerase system also suggest that ExuT is a membrane protein .
	manualset3
113908	3	402394	13	NULL	NULL	0	NULL	T7-RNA polymerase system	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Localization studies with the labeled polypeptide in the T7-RNA polymerase system also suggest that ExuT is a membrane protein .
	manualset3
113909	4	402394	13	NULL	NULL	0	NULL	ExuT	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Localization studies with the labeled polypeptide in the T7-RNA polymerase system also suggest that ExuT is a membrane protein .
	manualset3
113910	5	402394	13	NULL	NULL	0	NULL	membrane protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Localization studies with the labeled polypeptide in the T7-RNA polymerase system also suggest that ExuT is a membrane protein .
	manualset3
113911	1	402395	13	NULL	NULL	0	NULL	Localized immune memory	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Localized immune memory in the lung .
	manualset3
113912	2	402395	13	NULL	NULL	0	NULL	lung	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Localized immune memory in the lung .
	manualset3
113913	1	402396	13	NULL	NULL	0	NULL	Simvastatin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Locally applied Simvastatin improves fracture healing in mice .
	manualset3
113914	2	402396	13	NULL	NULL	0	NULL	fracture healing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Locally applied Simvastatin improves fracture healing in mice .
	manualset3
113915	3	402396	13	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Locally applied Simvastatin improves fracture healing in mice .
	manualset3
113916	1	402397	13	NULL	NULL	0	NULL	Locomotor movements	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Locomotor movements restricted to imposed ankle joint movements were followed by no , or only focal EMG responses in the stretched muscles .
	manualset3
113917	2	402397	13	NULL	NULL	0	NULL	 ankle joint movements	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Locomotor movements restricted to imposed ankle joint movements were followed by no , or only focal EMG responses in the stretched muscles .
	manualset3
113918	3	402397	13	NULL	NULL	0	NULL	focal EMG responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Locomotor movements restricted to imposed ankle joint movements were followed by no , or only focal EMG responses in the stretched muscles .
	manualset3
113919	4	402397	13	NULL	NULL	0	NULL	muscles 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Locomotor movements restricted to imposed ankle joint movements were followed by no , or only focal EMG responses in the stretched muscles .
	manualset3
113920	1	402398	13	NULL	NULL	0	NULL	Logical approach	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Logical approach to transplant patient monitoring .
	manualset3
113921	2	402398	13	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Logical approach to transplant patient monitoring .
	manualset3
113922	3	402398	13	NULL	NULL	0	NULL	monitoring	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Logical approach to transplant patient monitoring .
	manualset3
113923	1	402399	13	NULL	NULL	0	NULL	Logistic regression analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Logistic regression analyses were performed with 95 % confidence intervals and the odds ratio for fear-avoidance beliefs and ADL was 2.5 and for catastrophizing and pain 1.8 , both with confidence interval above unity .
	manualset3
113924	2	402399	13	NULL	NULL	0	NULL	95 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Logistic regression analyses were performed with 95 % confidence intervals and the odds ratio for fear-avoidance beliefs and ADL was 2.5 and for catastrophizing and pain 1.8 , both with confidence interval above unity .
	manualset3
113925	3	402399	13	NULL	NULL	0	NULL	confidence intervals	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Logistic regression analyses were performed with 95 % confidence intervals and the odds ratio for fear-avoidance beliefs and ADL was 2.5 and for catastrophizing and pain 1.8 , both with confidence interval above unity .
	manualset3
113926	4	402399	13	NULL	NULL	0	NULL	odds ratio	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Logistic regression analyses were performed with 95 % confidence intervals and the odds ratio for fear-avoidance beliefs and ADL was 2.5 and for catastrophizing and pain 1.8 , both with confidence interval above unity .
	manualset3
113927	5	402399	13	NULL	NULL	0	NULL	fear-avoidance beliefs	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Logistic regression analyses were performed with 95 % confidence intervals and the odds ratio for fear-avoidance beliefs and ADL was 2.5 and for catastrophizing and pain 1.8 , both with confidence interval above unity .
	manualset3
113928	6	402399	13	NULL	NULL	0	NULL	ADL 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Logistic regression analyses were performed with 95 % confidence intervals and the odds ratio for fear-avoidance beliefs and ADL was 2.5 and for catastrophizing and pain 1.8 , both with confidence interval above unity .
	manualset3
113929	7	402399	13	NULL	NULL	0	NULL	2.5	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Logistic regression analyses were performed with 95 % confidence intervals and the odds ratio for fear-avoidance beliefs and ADL was 2.5 and for catastrophizing and pain 1.8 , both with confidence interval above unity .
	manualset3
113930	8	402399	13	NULL	NULL	0	NULL	pain 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Logistic regression analyses were performed with 95 % confidence intervals and the odds ratio for fear-avoidance beliefs and ADL was 2.5 and for catastrophizing and pain 1.8 , both with confidence interval above unity .
	manualset3
113931	9	402399	13	NULL	NULL	0	NULL	1.8 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Logistic regression analyses were performed with 95 % confidence intervals and the odds ratio for fear-avoidance beliefs and ADL was 2.5 and for catastrophizing and pain 1.8 , both with confidence interval above unity .
	manualset3
113932	10	402399	13	NULL	NULL	0	NULL	confidence interval	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Logistic regression analyses were performed with 95 % confidence intervals and the odds ratio for fear-avoidance beliefs and ADL was 2.5 and for catastrophizing and pain 1.8 , both with confidence interval above unity .
	manualset3
113933	11	402399	13	NULL	NULL	0	NULL	above unity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Logistic regression analyses were performed with 95 % confidence intervals and the odds ratio for fear-avoidance beliefs and ADL was 2.5 and for catastrophizing and pain 1.8 , both with confidence interval above unity .
	manualset3
113934	1	402400	13	NULL	NULL	0	NULL	58-year-old woman 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A 58-year-old woman suspected of gallbladder carcinoma underwent laparoscopic cholecystectomy .
	manualset3
113935	2	402400	13	NULL	NULL	0	NULL	gallbladder carcinoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 58-year-old woman suspected of gallbladder carcinoma underwent laparoscopic cholecystectomy .
	manualset3
113936	3	402400	13	NULL	NULL	0	NULL	laparoscopic cholecystectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A 58-year-old woman suspected of gallbladder carcinoma underwent laparoscopic cholecystectomy .
	manualset3
113937	1	402401	13	NULL	NULL	NULL	NULL	Long-acting phosphodiesterase 5 inhibitor	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Long-acting phosphodiesterase 5 inhibitor , tadalafil , and superoxide dismutase mimetic , tempol , protect against acute hypoxia-induced pulmonary hypertension in rats .
	manualset3
113938	2	402401	13	NULL	NULL	0	NULL	tadalafil	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-acting phosphodiesterase 5 inhibitor , tadalafil , and superoxide dismutase mimetic , tempol , protect against acute hypoxia-induced pulmonary hypertension in rats .
	manualset3
113939	3	402401	13	NULL	NULL	0	NULL	superoxide dismutase mimetic	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-acting phosphodiesterase 5 inhibitor , tadalafil , and superoxide dismutase mimetic , tempol , protect against acute hypoxia-induced pulmonary hypertension in rats .
	manualset3
113940	4	402401	13	NULL	NULL	0	NULL	tempol 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-acting phosphodiesterase 5 inhibitor , tadalafil , and superoxide dismutase mimetic , tempol , protect against acute hypoxia-induced pulmonary hypertension in rats .
	manualset3
113941	5	402401	13	NULL	NULL	0	NULL	acute hypoxia-induced pulmonary hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-acting phosphodiesterase 5 inhibitor , tadalafil , and superoxide dismutase mimetic , tempol , protect against acute hypoxia-induced pulmonary hypertension in rats .
	manualset3
113942	6	402401	13	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-acting phosphodiesterase 5 inhibitor , tadalafil , and superoxide dismutase mimetic , tempol , protect against acute hypoxia-induced pulmonary hypertension in rats .
	manualset3
113943	1	402402	13	NULL	NULL	0	NULL	Long-term application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term application of lead arsenate in orchards has led to a significant accumulation of Pb and As in the topsoil .
	manualset3
113944	2	402402	13	NULL	NULL	0	NULL	lead arsenate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term application of lead arsenate in orchards has led to a significant accumulation of Pb and As in the topsoil .
	manualset3
113945	3	402402	13	NULL	NULL	0	NULL	orchards	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term application of lead arsenate in orchards has led to a significant accumulation of Pb and As in the topsoil .
	manualset3
113946	4	402402	13	NULL	NULL	0	NULL	accumulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term application of lead arsenate in orchards has led to a significant accumulation of Pb and As in the topsoil .
	manualset3
113947	5	402402	13	NULL	NULL	0	NULL	Pb	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term application of lead arsenate in orchards has led to a significant accumulation of Pb and As in the topsoil .
	manualset3
113948	6	402402	13	NULL	NULL	0	NULL	As	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term application of lead arsenate in orchards has led to a significant accumulation of Pb and As in the topsoil .
	manualset3
113949	7	402402	13	NULL	NULL	0	NULL	topsoil	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term application of lead arsenate in orchards has led to a significant accumulation of Pb and As in the topsoil .
	manualset3
113950	1	402403	13	NULL	NULL	0	NULL	Long-term effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term effects of highly selective vagotomy ( HSV ) in dogs on acid and pepsin secretion .
	manualset3
113951	2	402403	13	NULL	NULL	0	NULL	highly selective vagotomy ( HSV )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term effects of highly selective vagotomy ( HSV ) in dogs on acid and pepsin secretion .
	manualset3
113952	3	402403	13	NULL	NULL	0	NULL	dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term effects of highly selective vagotomy ( HSV ) in dogs on acid and pepsin secretion .
	manualset3
113953	4	402403	13	NULL	NULL	0	NULL	acid secretion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term effects of highly selective vagotomy ( HSV ) in dogs on acid and pepsin secretion .
	manualset3
113954	5	402403	13	NULL	NULL	0	NULL	pepsin secretion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term effects of highly selective vagotomy ( HSV ) in dogs on acid and pepsin secretion .
	manualset3
113955	1	402404	13	NULL	NULL	0	NULL	Long-term evaluation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term evaluation showed a high incidence of clicking and pain , not evident prior to surgery .
	manualset3
113956	2	402404	13	NULL	NULL	0	NULL	incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term evaluation showed a high incidence of clicking and pain , not evident prior to surgery .
	manualset3
113957	3	402404	13	NULL	NULL	0	NULL	clicking	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term evaluation showed a high incidence of clicking and pain , not evident prior to surgery .
	manualset3
113958	4	402404	13	NULL	NULL	0	NULL	pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term evaluation showed a high incidence of clicking and pain , not evident prior to surgery .
	manualset3
113959	5	402404	13	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term evaluation showed a high incidence of clicking and pain , not evident prior to surgery .
	manualset3
113960	1	402405	13	NULL	NULL	0	NULL	6.9-kb DNA fragment	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A 6.9-kb DNA fragment containing two mouse U1b genes was introduced by cotransfection with the Herpes simplex virus ( HSV ) thymidine kinase ( TK ) gene into tk - mouse L cells .
	manualset3
113961	2	402405	13	NULL	NULL	0	NULL	two mouse U1b genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A 6.9-kb DNA fragment containing two mouse U1b genes was introduced by cotransfection with the Herpes simplex virus ( HSV ) thymidine kinase ( TK ) gene into tk - mouse L cells .
	manualset3
113962	3	402405	13	NULL	NULL	0	NULL	cotransfection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A 6.9-kb DNA fragment containing two mouse U1b genes was introduced by cotransfection with the Herpes simplex virus ( HSV ) thymidine kinase ( TK ) gene into tk - mouse L cells .
	manualset3
113963	4	402405	13	NULL	NULL	0	NULL	Herpes simplex virus ( HSV ) thymidine kinase ( TK ) gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A 6.9-kb DNA fragment containing two mouse U1b genes was introduced by cotransfection with the Herpes simplex virus ( HSV ) thymidine kinase ( TK ) gene into tk - mouse L cells .
	manualset3
113964	5	402405	13	NULL	NULL	0	NULL	tk - mouse L cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A 6.9-kb DNA fragment containing two mouse U1b genes was introduced by cotransfection with the Herpes simplex virus ( HSV ) thymidine kinase ( TK ) gene into tk - mouse L cells .
	manualset3
113965	1	402406	13	NULL	NULL	0	NULL	Long-term medical management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term medical management of PD is frequently complicated by fluctuating motor functions and dyskinesias .
	manualset3
113966	2	402406	13	NULL	NULL	0	NULL	PD 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term medical management of PD is frequently complicated by fluctuating motor functions and dyskinesias .
	manualset3
113967	3	402406	13	NULL	NULL	0	NULL	motor functions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term medical management of PD is frequently complicated by fluctuating motor functions and dyskinesias .
	manualset3
113968	4	402406	13	NULL	NULL	0	NULL	dyskinesias	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term medical management of PD is frequently complicated by fluctuating motor functions and dyskinesias .
	manualset3
113969	1	402407	13	NULL	NULL	0	NULL	Long-term outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term outcome after coil embolization of cavernous sinus arteriovenous fistulas .
	manualset3
113970	2	402407	13	NULL	NULL	0	NULL	coil embolization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term outcome after coil embolization of cavernous sinus arteriovenous fistulas .
	manualset3
113971	3	402407	13	NULL	NULL	0	NULL	cavernous sinus arteriovenous fistulas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term outcome after coil embolization of cavernous sinus arteriovenous fistulas .
	manualset3
113972	1	402408	13	NULL	NULL	0	NULL	Long-term outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term outcome of comprehensive central compartment dissection in patients with recurrent/persistent papillary thyroid carcinoma .
	manualset3
113973	2	402408	13	NULL	NULL	0	NULL	compartment dissection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term outcome of comprehensive central compartment dissection in patients with recurrent/persistent papillary thyroid carcinoma .
	manualset3
113974	3	402408	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term outcome of comprehensive central compartment dissection in patients with recurrent/persistent papillary thyroid carcinoma .
	manualset3
113975	4	402408	13	NULL	NULL	0	NULL	recurrent/persistent papillary thyroid carcinoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term outcome of comprehensive central compartment dissection in patients with recurrent/persistent papillary thyroid carcinoma .
	manualset3
113976	1	402409	13	NULL	NULL	0	NULL	Long-term potentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term potentiation could still be induced in the presence of calyculin A , but the effect of the compound was slightly reduced on potentiated compared with control pathways .
	manualset3
113977	2	402409	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term potentiation could still be induced in the presence of calyculin A , but the effect of the compound was slightly reduced on potentiated compared with control pathways .
	manualset3
113979	3	402409	13	NULL	NULL	0	NULL	calyculin A	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term potentiation could still be induced in the presence of calyculin A , but the effect of the compound was slightly reduced on potentiated compared with control pathways .
	manualset3
113981	4	402409	13	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term potentiation could still be induced in the presence of calyculin A , but the effect of the compound was slightly reduced on potentiated compared with control pathways .
	manualset3
113983	5	402409	13	NULL	NULL	0	NULL	compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term potentiation could still be induced in the presence of calyculin A , but the effect of the compound was slightly reduced on potentiated compared with control pathways .
	manualset3
113985	6	402409	13	NULL	NULL	0	NULL	control pathways 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term potentiation could still be induced in the presence of calyculin A , but the effect of the compound was slightly reduced on potentiated compared with control pathways .
	manualset3
113988	1	402410	13	NULL	NULL	0	NULL	Long-term prospective analyses	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term prospective analyses will be critical in determining the role of UKA as a mainstay in the treatment of single compartment knee degenerative joint disease .
	manualset3
113989	2	402410	13	NULL	NULL	0	NULL	role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term prospective analyses will be critical in determining the role of UKA as a mainstay in the treatment of single compartment knee degenerative joint disease .
	manualset3
113990	3	402410	13	NULL	NULL	0	NULL	UKA 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term prospective analyses will be critical in determining the role of UKA as a mainstay in the treatment of single compartment knee degenerative joint disease .
	manualset3
113991	4	402410	13	NULL	NULL	0	NULL	mainstay	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term prospective analyses will be critical in determining the role of UKA as a mainstay in the treatment of single compartment knee degenerative joint disease .
	manualset3
113992	5	402410	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term prospective analyses will be critical in determining the role of UKA as a mainstay in the treatment of single compartment knee degenerative joint disease .
	manualset3
113993	6	402410	13	NULL	NULL	0	NULL	single compartment knee degenerative joint disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term prospective analyses will be critical in determining the role of UKA as a mainstay in the treatment of single compartment knee degenerative joint disease .
	manualset3
113994	1	402411	13	NULL	NULL	0	NULL	Long-term study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term study of fluvoxamine : a new rapid-acting antidepressant .
	manualset3
113995	2	402411	13	NULL	NULL	0	NULL	fluvoxamine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term study of fluvoxamine : a new rapid-acting antidepressant .
	manualset3
113996	3	402411	13	NULL	NULL	0	NULL	rapid-acting antidepressant 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term study of fluvoxamine : a new rapid-acting antidepressant .
	manualset3
114007	1	402412	13	NULL	NULL	0	NULL	Long-term subdural video/electroencephalographic ( EEG ) monitoring 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term subdural video/electroencephalographic ( EEG ) monitoring was performed in a series of patients with medically intractable complex partial seizures , in a study of diagnostic accuracy , to test the hypothesis that the time from ictal subdural EEG seizure onset to clinical seizure onset ( ECOT ) is correlated with temporal lobe epileptogenicity and confirm measures of validity of ECOT for predicting seizure-free outcome following anterior temporal lobectomy and amygdalohippocampectomy ( ATL/AH ) .
	manualset3
114009	2	402412	13	NULL	NULL	0	NULL	series of patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term subdural video/electroencephalographic ( EEG ) monitoring was performed in a series of patients with medically intractable complex partial seizures , in a study of diagnostic accuracy , to test the hypothesis that the time from ictal subdural EEG seizure onset to clinical seizure onset ( ECOT ) is correlated with temporal lobe epileptogenicity and confirm measures of validity of ECOT for predicting seizure-free outcome following anterior temporal lobectomy and amygdalohippocampectomy ( ATL/AH ) .
	manualset3
114013	3	402412	13	NULL	NULL	0	NULL	partial seizures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term subdural video/electroencephalographic ( EEG ) monitoring was performed in a series of patients with medically intractable complex partial seizures , in a study of diagnostic accuracy , to test the hypothesis that the time from ictal subdural EEG seizure onset to clinical seizure onset ( ECOT ) is correlated with temporal lobe epileptogenicity and confirm measures of validity of ECOT for predicting seizure-free outcome following anterior temporal lobectomy and amygdalohippocampectomy ( ATL/AH ) .
	manualset3
114014	4	402412	13	NULL	NULL	0	NULL	study of diagnostic accuracy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term subdural video/electroencephalographic ( EEG ) monitoring was performed in a series of patients with medically intractable complex partial seizures , in a study of diagnostic accuracy , to test the hypothesis that the time from ictal subdural EEG seizure onset to clinical seizure onset ( ECOT ) is correlated with temporal lobe epileptogenicity and confirm measures of validity of ECOT for predicting seizure-free outcome following anterior temporal lobectomy and amygdalohippocampectomy ( ATL/AH ) .
	manualset3
114015	5	402412	13	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term subdural video/electroencephalographic ( EEG ) monitoring was performed in a series of patients with medically intractable complex partial seizures , in a study of diagnostic accuracy , to test the hypothesis that the time from ictal subdural EEG seizure onset to clinical seizure onset ( ECOT ) is correlated with temporal lobe epileptogenicity and confirm measures of validity of ECOT for predicting seizure-free outcome following anterior temporal lobectomy and amygdalohippocampectomy ( ATL/AH ) .
	manualset3
114016	6	402412	13	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term subdural video/electroencephalographic ( EEG ) monitoring was performed in a series of patients with medically intractable complex partial seizures , in a study of diagnostic accuracy , to test the hypothesis that the time from ictal subdural EEG seizure onset to clinical seizure onset ( ECOT ) is correlated with temporal lobe epileptogenicity and confirm measures of validity of ECOT for predicting seizure-free outcome following anterior temporal lobectomy and amygdalohippocampectomy ( ATL/AH ) .
	manualset3
114018	7	402412	13	NULL	NULL	0	NULL	 ictal subdural EEG seizure onset	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term subdural video/electroencephalographic ( EEG ) monitoring was performed in a series of patients with medically intractable complex partial seizures , in a study of diagnostic accuracy , to test the hypothesis that the time from ictal subdural EEG seizure onset to clinical seizure onset ( ECOT ) is correlated with temporal lobe epileptogenicity and confirm measures of validity of ECOT for predicting seizure-free outcome following anterior temporal lobectomy and amygdalohippocampectomy ( ATL/AH ) .
	manualset3
114020	8	402412	13	NULL	NULL	0	NULL	clinical seizure onset ( ECOT ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term subdural video/electroencephalographic ( EEG ) monitoring was performed in a series of patients with medically intractable complex partial seizures , in a study of diagnostic accuracy , to test the hypothesis that the time from ictal subdural EEG seizure onset to clinical seizure onset ( ECOT ) is correlated with temporal lobe epileptogenicity and confirm measures of validity of ECOT for predicting seizure-free outcome following anterior temporal lobectomy and amygdalohippocampectomy ( ATL/AH ) .
	manualset3
114021	9	402412	13	NULL	NULL	0	NULL	temporal lobe 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term subdural video/electroencephalographic ( EEG ) monitoring was performed in a series of patients with medically intractable complex partial seizures , in a study of diagnostic accuracy , to test the hypothesis that the time from ictal subdural EEG seizure onset to clinical seizure onset ( ECOT ) is correlated with temporal lobe epileptogenicity and confirm measures of validity of ECOT for predicting seizure-free outcome following anterior temporal lobectomy and amygdalohippocampectomy ( ATL/AH ) .
	manualset3
114023	10	402412	13	NULL	NULL	0	NULL	epileptogenicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term subdural video/electroencephalographic ( EEG ) monitoring was performed in a series of patients with medically intractable complex partial seizures , in a study of diagnostic accuracy , to test the hypothesis that the time from ictal subdural EEG seizure onset to clinical seizure onset ( ECOT ) is correlated with temporal lobe epileptogenicity and confirm measures of validity of ECOT for predicting seizure-free outcome following anterior temporal lobectomy and amygdalohippocampectomy ( ATL/AH ) .
	manualset3
114025	11	402412	13	NULL	NULL	0	NULL	measures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term subdural video/electroencephalographic ( EEG ) monitoring was performed in a series of patients with medically intractable complex partial seizures , in a study of diagnostic accuracy , to test the hypothesis that the time from ictal subdural EEG seizure onset to clinical seizure onset ( ECOT ) is correlated with temporal lobe epileptogenicity and confirm measures of validity of ECOT for predicting seizure-free outcome following anterior temporal lobectomy and amygdalohippocampectomy ( ATL/AH ) .
	manualset3
114027	12	402412	13	NULL	NULL	0	NULL	validity of ECOT	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term subdural video/electroencephalographic ( EEG ) monitoring was performed in a series of patients with medically intractable complex partial seizures , in a study of diagnostic accuracy , to test the hypothesis that the time from ictal subdural EEG seizure onset to clinical seizure onset ( ECOT ) is correlated with temporal lobe epileptogenicity and confirm measures of validity of ECOT for predicting seizure-free outcome following anterior temporal lobectomy and amygdalohippocampectomy ( ATL/AH ) .
	manualset3
114029	13	402412	13	NULL	NULL	0	NULL	seizure-free outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term subdural video/electroencephalographic ( EEG ) monitoring was performed in a series of patients with medically intractable complex partial seizures , in a study of diagnostic accuracy , to test the hypothesis that the time from ictal subdural EEG seizure onset to clinical seizure onset ( ECOT ) is correlated with temporal lobe epileptogenicity and confirm measures of validity of ECOT for predicting seizure-free outcome following anterior temporal lobectomy and amygdalohippocampectomy ( ATL/AH ) .
	manualset3
114030	14	402412	13	NULL	NULL	0	NULL	anterior temporal lobectomy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term subdural video/electroencephalographic ( EEG ) monitoring was performed in a series of patients with medically intractable complex partial seizures , in a study of diagnostic accuracy , to test the hypothesis that the time from ictal subdural EEG seizure onset to clinical seizure onset ( ECOT ) is correlated with temporal lobe epileptogenicity and confirm measures of validity of ECOT for predicting seizure-free outcome following anterior temporal lobectomy and amygdalohippocampectomy ( ATL/AH ) .
	manualset3
114031	15	402412	13	NULL	NULL	0	NULL	amygdalohippocampectomy ( ATL/AH ) 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term subdural video/electroencephalographic ( EEG ) monitoring was performed in a series of patients with medically intractable complex partial seizures , in a study of diagnostic accuracy , to test the hypothesis that the time from ictal subdural EEG seizure onset to clinical seizure onset ( ECOT ) is correlated with temporal lobe epileptogenicity and confirm measures of validity of ECOT for predicting seizure-free outcome following anterior temporal lobectomy and amygdalohippocampectomy ( ATL/AH ) .
	manualset3
114035	1	402413	13	NULL	NULL	0	NULL	Long-term treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term treatment with mirtazapine increases FT3 levels and decreases FT4 maybe involving the deiodination process of T4 into T3 .
	manualset3
114036	2	402413	13	NULL	NULL	0	NULL	mirtazapine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term treatment with mirtazapine increases FT3 levels and decreases FT4 maybe involving the deiodination process of T4 into T3 .
	manualset3
114039	4	402413	13	NULL	NULL	0	NULL	FT3 levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term treatment with mirtazapine increases FT3 levels and decreases FT4 maybe involving the deiodination process of T4 into T3 .
	manualset3
114041	6	402413	13	NULL	NULL	0	NULL	FT4	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term treatment with mirtazapine increases FT3 levels and decreases FT4 maybe involving the deiodination process of T4 into T3 .
	manualset3
114042	7	402413	13	NULL	NULL	NULL	NULL	deiodination process	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Long-term treatment with mirtazapine increases FT3 levels and decreases FT4 maybe involving the deiodination process of T4 into T3 .
	manualset3
114043	8	402413	13	NULL	NULL	0	NULL	T4	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term treatment with mirtazapine increases FT3 levels and decreases FT4 maybe involving the deiodination process of T4 into T3 .
	manualset3
114044	9	402413	13	NULL	NULL	0	NULL	T3	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term treatment with mirtazapine increases FT3 levels and decreases FT4 maybe involving the deiodination process of T4 into T3 .
	manualset3
114048	1	402414	13	NULL	NULL	0	NULL	61-year-old man	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A 61-year-old man underwent amputation of the rectum for advanced lower rectal cancer in April 2005 .
	manualset3
114051	2	402414	13	NULL	NULL	0	NULL	amputation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A 61-year-old man underwent amputation of the rectum for advanced lower rectal cancer in April 2005 .
	manualset3
114052	3	402414	13	NULL	NULL	0	NULL	rectum 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A 61-year-old man underwent amputation of the rectum for advanced lower rectal cancer in April 2005 .
	manualset3
114053	4	402414	13	NULL	NULL	0	NULL	lower rectal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A 61-year-old man underwent amputation of the rectum for advanced lower rectal cancer in April 2005 .
	manualset3
114055	5	402414	13	NULL	NULL	0	NULL	April 2005	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	A 61-year-old man underwent amputation of the rectum for advanced lower rectal cancer in April 2005 .
	manualset3
114060	1	402415	13	NULL	NULL	0	NULL	wine consumption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term wine consumption is related to cardiovascular mortality and life expectancy independently of moderate alcohol intake : the Zutphen Study .
	manualset3
114061	2	402415	13	NULL	NULL	0	NULL	cardiovascular mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term wine consumption is related to cardiovascular mortality and life expectancy independently of moderate alcohol intake : the Zutphen Study .
	manualset3
114062	3	402415	13	NULL	NULL	0	NULL	life expectancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term wine consumption is related to cardiovascular mortality and life expectancy independently of moderate alcohol intake : the Zutphen Study .
	manualset3
114063	4	402415	13	NULL	NULL	0	NULL	alcohol intake	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term wine consumption is related to cardiovascular mortality and life expectancy independently of moderate alcohol intake : the Zutphen Study .
	manualset3
114064	5	402415	13	NULL	NULL	0	NULL	Zutphen Study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term wine consumption is related to cardiovascular mortality and life expectancy independently of moderate alcohol intake : the Zutphen Study .
	manualset3
114065	1	402416	13	NULL	NULL	0	NULL	Long term survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Long term survival following methotrexate treatment .
	manualset3
114066	2	402416	13	NULL	NULL	0	NULL	methotrexate	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Long term survival following methotrexate treatment .
	manualset3
114067	3	402416	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Long term survival following methotrexate treatment .
	manualset3
114068	1	402417	13	NULL	NULL	NULL	NULL	Long term survival 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Long term survival of allografted muscle precursor cells following a limited period of treatment with cyclosporin A .
	manualset3
114069	2	402417	13	NULL	NULL	0	NULL	muscle precursor cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Long term survival of allografted muscle precursor cells following a limited period of treatment with cyclosporin A .
	manualset3
114070	3	402417	13	NULL	NULL	0	NULL	period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Long term survival of allografted muscle precursor cells following a limited period of treatment with cyclosporin A .
	manualset3
114071	4	402417	13	NULL	NULL	0	NULL	treatment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Long term survival of allografted muscle precursor cells following a limited period of treatment with cyclosporin A .
	manualset3
114072	5	402417	13	NULL	NULL	0	NULL	cyclosporin A	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Long term survival of allografted muscle precursor cells following a limited period of treatment with cyclosporin A .
	manualset3
114073	1	402418	13	NULL	NULL	0	NULL	Longer nerve compression time	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Longer nerve compression time and sustained , decreased muscle power with signs of active denervation in EMG are indicators of poor prognosis .
	manualset3
114074	2	402418	13	NULL	NULL	0	NULL	muscle power 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Longer nerve compression time and sustained , decreased muscle power with signs of active denervation in EMG are indicators of poor prognosis .
	manualset3
114075	3	402418	13	NULL	NULL	0	NULL	signs of active denervation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Longer nerve compression time and sustained , decreased muscle power with signs of active denervation in EMG are indicators of poor prognosis .
	manualset3
114076	4	402418	13	NULL	NULL	NULL	NULL	EMG	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Longer nerve compression time and sustained , decreased muscle power with signs of active denervation in EMG are indicators of poor prognosis .
	manualset3
114077	5	402418	13	NULL	NULL	0	NULL	indicators	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Longer nerve compression time and sustained , decreased muscle power with signs of active denervation in EMG are indicators of poor prognosis .
	manualset3
114078	6	402418	13	NULL	NULL	0	NULL	prognosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Longer nerve compression time and sustained , decreased muscle power with signs of active denervation in EMG are indicators of poor prognosis .
	manualset3
114079	1	402419	13	NULL	NULL	0	NULL	Longevity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Longevity , fecundity , and egg fertility were examined for female/male pairs of moths maintained with the following food regimens : water , sucrose water , honey water , apple juice , apple flesh , or starved , i.e. , no food or water provided .
	manualset3
114080	2	402419	13	NULL	NULL	0	NULL	fecundity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Longevity , fecundity , and egg fertility were examined for female/male pairs of moths maintained with the following food regimens : water , sucrose water , honey water , apple juice , apple flesh , or starved , i.e. , no food or water provided .
	manualset3
114081	3	402419	13	NULL	NULL	0	NULL	egg fertility 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Longevity , fecundity , and egg fertility were examined for female/male pairs of moths maintained with the following food regimens : water , sucrose water , honey water , apple juice , apple flesh , or starved , i.e. , no food or water provided .
	manualset3
114082	4	402419	13	NULL	NULL	0	NULL	female/male pairs of moths	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Longevity , fecundity , and egg fertility were examined for female/male pairs of moths maintained with the following food regimens : water , sucrose water , honey water , apple juice , apple flesh , or starved , i.e. , no food or water provided .
	manualset3
114083	5	402419	13	NULL	NULL	0	NULL	food regimens	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Longevity , fecundity , and egg fertility were examined for female/male pairs of moths maintained with the following food regimens : water , sucrose water , honey water , apple juice , apple flesh , or starved , i.e. , no food or water provided .
	manualset3
114084	6	402419	13	NULL	NULL	NULL	NULL	water	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Longevity , fecundity , and egg fertility were examined for female/male pairs of moths maintained with the following food regimens : water , sucrose water , honey water , apple juice , apple flesh , or starved , i.e. , no food or water provided .
	manualset3
114085	7	402419	13	NULL	NULL	0	NULL	sucrose water	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Longevity , fecundity , and egg fertility were examined for female/male pairs of moths maintained with the following food regimens : water , sucrose water , honey water , apple juice , apple flesh , or starved , i.e. , no food or water provided .
	manualset3
114086	8	402419	13	NULL	NULL	0	NULL	honey water 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Longevity , fecundity , and egg fertility were examined for female/male pairs of moths maintained with the following food regimens : water , sucrose water , honey water , apple juice , apple flesh , or starved , i.e. , no food or water provided .
	manualset3
114087	9	402419	13	NULL	NULL	0	NULL	apple juice 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Longevity , fecundity , and egg fertility were examined for female/male pairs of moths maintained with the following food regimens : water , sucrose water , honey water , apple juice , apple flesh , or starved , i.e. , no food or water provided .
	manualset3
114088	10	402419	13	NULL	NULL	0	NULL	apple flesh	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Longevity , fecundity , and egg fertility were examined for female/male pairs of moths maintained with the following food regimens : water , sucrose water , honey water , apple juice , apple flesh , or starved , i.e. , no food or water provided .
	manualset3
114089	11	402419	13	NULL	NULL	0	NULL	food	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Longevity , fecundity , and egg fertility were examined for female/male pairs of moths maintained with the following food regimens : water , sucrose water , honey water , apple juice , apple flesh , or starved , i.e. , no food or water provided .
	manualset3
114090	12	402419	13	NULL	NULL	NULL	NULL	water	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Longevity , fecundity , and egg fertility were examined for female/male pairs of moths maintained with the following food regimens : water , sucrose water , honey water , apple juice , apple flesh , or starved , i.e. , no food or water provided .
	manualset3
114091	1	402420	13	NULL	NULL	0	NULL	Longitudinal effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Longitudinal effects of prenatal cocaine use on mother-child interactions at ages 3 and 5 years .
	manualset3
114092	2	402420	13	NULL	NULL	0	NULL	prenatal cocaine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Longitudinal effects of prenatal cocaine use on mother-child interactions at ages 3 and 5 years .
	manualset3
114093	3	402420	13	NULL	NULL	0	NULL	mother-child interactions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Longitudinal effects of prenatal cocaine use on mother-child interactions at ages 3 and 5 years .
	manualset3
114094	4	402420	13	NULL	NULL	0	NULL	age 3 years	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Longitudinal effects of prenatal cocaine use on mother-child interactions at ages 3 and 5 years .
	manualset3
114095	5	402420	13	NULL	NULL	0	NULL	age 5 years	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Longitudinal effects of prenatal cocaine use on mother-child interactions at ages 3 and 5 years .
	manualset3
114096	1	402421	13	NULL	NULL	0	NULL	Longspurs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Longspurs and snow buntings : phylogeny and biogeography of a high-latitude clade ( Calcarius ) .
	manualset3
114097	2	402421	13	NULL	NULL	0	NULL	snow buntings	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Longspurs and snow buntings : phylogeny and biogeography of a high-latitude clade ( Calcarius ) .
	manualset3
114098	3	402421	13	NULL	NULL	0	NULL	phylogeny	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Longspurs and snow buntings : phylogeny and biogeography of a high-latitude clade ( Calcarius ) .
	manualset3
114099	4	402421	13	NULL	NULL	0	NULL	biogeography	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Longspurs and snow buntings : phylogeny and biogeography of a high-latitude clade ( Calcarius ) .
	manualset3
114100	5	402421	13	NULL	NULL	0	NULL	high-latitude clade ( Calcarius ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Longspurs and snow buntings : phylogeny and biogeography of a high-latitude clade ( Calcarius ) .
	manualset3
114101	1	402422	13	NULL	NULL	0	NULL	Lonomycin A	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Lonomycin A increased developed and resting tensions in Tyrode solution containing 1.8 mM Ca2 + .
	manualset3
114102	2	402422	13	NULL	NULL	0	NULL	tensions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Lonomycin A increased developed and resting tensions in Tyrode solution containing 1.8 mM Ca2 + .
	manualset3
114103	3	402422	13	NULL	NULL	0	NULL	Tyrode solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lonomycin A increased developed and resting tensions in Tyrode solution containing 1.8 mM Ca2 + .
	manualset3
114104	4	402422	13	NULL	NULL	0	NULL	1.8 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Lonomycin A increased developed and resting tensions in Tyrode solution containing 1.8 mM Ca2 + .
	manualset3
114105	5	402422	13	NULL	NULL	0	NULL	Ca2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Lonomycin A increased developed and resting tensions in Tyrode solution containing 1.8 mM Ca2 + .
	manualset3
114106	1	402423	13	NULL	NULL	0	NULL	62-year-old man	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A 62-year-old man experienced double vision in his left eye from December 2008 and received a diagnosis of diabetic neuropathy .
	manualset3
114107	2	402423	13	NULL	NULL	0	NULL	double vision	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 62-year-old man experienced double vision in his left eye from December 2008 and received a diagnosis of diabetic neuropathy .
	manualset3
114108	3	402423	13	NULL	NULL	0	NULL	left eye	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A 62-year-old man experienced double vision in his left eye from December 2008 and received a diagnosis of diabetic neuropathy .
	manualset3
114109	4	402423	13	NULL	NULL	0	NULL	December 2008	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	A 62-year-old man experienced double vision in his left eye from December 2008 and received a diagnosis of diabetic neuropathy .
	manualset3
114110	5	402423	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A 62-year-old man experienced double vision in his left eye from December 2008 and received a diagnosis of diabetic neuropathy .
	manualset3
114111	6	402423	13	NULL	NULL	0	NULL	diabetic neuropathy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 62-year-old man experienced double vision in his left eye from December 2008 and received a diagnosis of diabetic neuropathy .
	manualset3
114112	1	402424	13	NULL	NULL	0	NULL	location	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Looking at the location of the new neurons , we found that while in control animals 76 % of them had migrated to the granule cell layer , in isolated animals only 55 % of the new neurons had reached this layer .
	manualset3
114113	2	402424	13	NULL	NULL	0	NULL	new neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Looking at the location of the new neurons , we found that while in control animals 76 % of them had migrated to the granule cell layer , in isolated animals only 55 % of the new neurons had reached this layer .
	manualset3
114114	3	402424	13	NULL	NULL	0	NULL	control animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Looking at the location of the new neurons , we found that while in control animals 76 % of them had migrated to the granule cell layer , in isolated animals only 55 % of the new neurons had reached this layer .
	manualset3
114115	4	402424	13	NULL	NULL	0	NULL	76 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Looking at the location of the new neurons , we found that while in control animals 76 % of them had migrated to the granule cell layer , in isolated animals only 55 % of the new neurons had reached this layer .
	manualset3
114116	5	402424	13	NULL	NULL	NULL	NULL	granule cell layer	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Looking at the location of the new neurons , we found that while in control animals 76 % of them had migrated to the granule cell layer , in isolated animals only 55 % of the new neurons had reached this layer .
	manualset3
114117	6	402424	13	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Looking at the location of the new neurons , we found that while in control animals 76 % of them had migrated to the granule cell layer , in isolated animals only 55 % of the new neurons had reached this layer .
	manualset3
114118	7	402424	13	NULL	NULL	0	NULL	55 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Looking at the location of the new neurons , we found that while in control animals 76 % of them had migrated to the granule cell layer , in isolated animals only 55 % of the new neurons had reached this layer .
	manualset3
114119	8	402424	13	NULL	NULL	0	NULL	new neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Looking at the location of the new neurons , we found that while in control animals 76 % of them had migrated to the granule cell layer , in isolated animals only 55 % of the new neurons had reached this layer .
	manualset3
114120	9	402424	13	NULL	NULL	NULL	NULL	layer	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Looking at the location of the new neurons , we found that while in control animals 76 % of them had migrated to the granule cell layer , in isolated animals only 55 % of the new neurons had reached this layer .
	manualset3
114121	1	402425	13	NULL	NULL	0	NULL	beamstop	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Looking behind the beamstop : X-ray solution scattering studies of structure and conformational changes of biological macromolecules .
	manualset3
114122	2	402425	13	NULL	NULL	0	NULL	X-ray solution scattering studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Looking behind the beamstop : X-ray solution scattering studies of structure and conformational changes of biological macromolecules .
	manualset3
114123	3	402425	13	NULL	NULL	0	NULL	structure	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Looking behind the beamstop : X-ray solution scattering studies of structure and conformational changes of biological macromolecules .
	manualset3
114124	4	402425	13	NULL	NULL	0	NULL	conformational changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Looking behind the beamstop : X-ray solution scattering studies of structure and conformational changes of biological macromolecules .
	manualset3
114125	5	402425	13	NULL	NULL	0	NULL	biological macromolecules 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Looking behind the beamstop : X-ray solution scattering studies of structure and conformational changes of biological macromolecules .
	manualset3
114126	1	402426	13	NULL	NULL	0	NULL	Loss -of-function mutations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss - and gain-of-function mutations in the broadly expressed gene Lrp5 affect bone formation , causing osteoporosis and high bone mass , respectively .
	manualset3
114127	2	402426	13	NULL	NULL	0	NULL	gain-of-function mutations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss - and gain-of-function mutations in the broadly expressed gene Lrp5 affect bone formation , causing osteoporosis and high bone mass , respectively .
	manualset3
114128	3	402426	13	NULL	NULL	0	NULL	gene Lrp5 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss - and gain-of-function mutations in the broadly expressed gene Lrp5 affect bone formation , causing osteoporosis and high bone mass , respectively .
	manualset3
114129	4	402426	13	NULL	NULL	0	NULL	bone formation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss - and gain-of-function mutations in the broadly expressed gene Lrp5 affect bone formation , causing osteoporosis and high bone mass , respectively .
	manualset3
114130	5	402426	13	NULL	NULL	0	NULL	osteoporosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss - and gain-of-function mutations in the broadly expressed gene Lrp5 affect bone formation , causing osteoporosis and high bone mass , respectively .
	manualset3
114131	6	402426	13	NULL	NULL	0	NULL	high bone mass	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss - and gain-of-function mutations in the broadly expressed gene Lrp5 affect bone formation , causing osteoporosis and high bone mass , respectively .
	manualset3
114132	1	402427	13	NULL	NULL	0	NULL	Loss	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of Abf2p , an abundant mitochondrial nucleoid-associated protein , results in increased mitochondrial frameshifts and direct-repeat mediated deletions but has no effect on the rate of mitochondrial point mutations .
	manualset3
114133	2	402427	13	NULL	NULL	0	NULL	Abf2p	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of Abf2p , an abundant mitochondrial nucleoid-associated protein , results in increased mitochondrial frameshifts and direct-repeat mediated deletions but has no effect on the rate of mitochondrial point mutations .
	manualset3
114134	3	402427	13	NULL	NULL	0	NULL	mitochondrial nucleoid-associated protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of Abf2p , an abundant mitochondrial nucleoid-associated protein , results in increased mitochondrial frameshifts and direct-repeat mediated deletions but has no effect on the rate of mitochondrial point mutations .
	manualset3
114135	4	402427	13	NULL	NULL	0	NULL	results 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of Abf2p , an abundant mitochondrial nucleoid-associated protein , results in increased mitochondrial frameshifts and direct-repeat mediated deletions but has no effect on the rate of mitochondrial point mutations .
	manualset3
114136	5	402427	13	NULL	NULL	0	NULL	mitochondrial frameshifts	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of Abf2p , an abundant mitochondrial nucleoid-associated protein , results in increased mitochondrial frameshifts and direct-repeat mediated deletions but has no effect on the rate of mitochondrial point mutations .
	manualset3
114137	6	402427	13	NULL	NULL	0	NULL	deletions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of Abf2p , an abundant mitochondrial nucleoid-associated protein , results in increased mitochondrial frameshifts and direct-repeat mediated deletions but has no effect on the rate of mitochondrial point mutations .
	manualset3
114138	7	402427	13	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of Abf2p , an abundant mitochondrial nucleoid-associated protein , results in increased mitochondrial frameshifts and direct-repeat mediated deletions but has no effect on the rate of mitochondrial point mutations .
	manualset3
114139	8	402427	13	NULL	NULL	0	NULL	rate of mitochondrial point mutations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of Abf2p , an abundant mitochondrial nucleoid-associated protein , results in increased mitochondrial frameshifts and direct-repeat mediated deletions but has no effect on the rate of mitochondrial point mutations .
	manualset3
114140	1	402428	13	NULL	NULL	0	NULL	Loss	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of CO2 to the atmosphere from biological fluids that are bicarbonate buffered resulted in a shift to alkaline pH by as much as 1 pH unit .
	manualset3
114141	2	402428	13	NULL	NULL	0	NULL	CO2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of CO2 to the atmosphere from biological fluids that are bicarbonate buffered resulted in a shift to alkaline pH by as much as 1 pH unit .
	manualset3
114142	3	402428	13	NULL	NULL	0	NULL	atmosphere 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of CO2 to the atmosphere from biological fluids that are bicarbonate buffered resulted in a shift to alkaline pH by as much as 1 pH unit .
	manualset3
114143	4	402428	13	NULL	NULL	0	NULL	biological fluids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of CO2 to the atmosphere from biological fluids that are bicarbonate buffered resulted in a shift to alkaline pH by as much as 1 pH unit .
	manualset3
114144	5	402428	13	NULL	NULL	0	NULL	bicarbonate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of CO2 to the atmosphere from biological fluids that are bicarbonate buffered resulted in a shift to alkaline pH by as much as 1 pH unit .
	manualset3
114145	6	402428	13	NULL	NULL	0	NULL	shift	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of CO2 to the atmosphere from biological fluids that are bicarbonate buffered resulted in a shift to alkaline pH by as much as 1 pH unit .
	manualset3
114146	7	402428	13	NULL	NULL	0	NULL	alkaline pH	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of CO2 to the atmosphere from biological fluids that are bicarbonate buffered resulted in a shift to alkaline pH by as much as 1 pH unit .
	manualset3
114147	8	402428	13	NULL	NULL	0	NULL	1 pH unit	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of CO2 to the atmosphere from biological fluids that are bicarbonate buffered resulted in a shift to alkaline pH by as much as 1 pH unit .
	manualset3
114148	1	402429	13	NULL	NULL	0	NULL	Loss	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of cardiac microRNA-mediated regulation leads to dilated cardiomyopathy and heart failure .
	manualset3
114149	2	402429	13	NULL	NULL	0	NULL	cardiac microRNA-mediated regulation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of cardiac microRNA-mediated regulation leads to dilated cardiomyopathy and heart failure .
	manualset3
114150	3	402429	13	NULL	NULL	0	NULL	 dilated cardiomyopathy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of cardiac microRNA-mediated regulation leads to dilated cardiomyopathy and heart failure .
	manualset3
114151	4	402429	13	NULL	NULL	0	NULL	heart failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of cardiac microRNA-mediated regulation leads to dilated cardiomyopathy and heart failure .
	manualset3
114152	1	402430	13	NULL	NULL	0	NULL	Loss 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of heterozygosity on chromosomes 10q , 9p , 17p and 13q in malays with malignant glioma .
	manualset3
114153	2	402430	13	NULL	NULL	0	NULL	 heterozygosity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of heterozygosity on chromosomes 10q , 9p , 17p and 13q in malays with malignant glioma .
	manualset3
114154	3	402430	13	NULL	NULL	NULL	NULL	chromosome 10q	Chromosome												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Loss of heterozygosity on chromosomes 10q , 9p , 17p and 13q in malays with malignant glioma .
	manualset3
114155	4	402430	13	NULL	NULL	0	NULL	chromosome 9p	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of heterozygosity on chromosomes 10q , 9p , 17p and 13q in malays with malignant glioma .
	manualset3
114156	5	402430	13	NULL	NULL	0	NULL	chromosome 17p	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of heterozygosity on chromosomes 10q , 9p , 17p and 13q in malays with malignant glioma .
	manualset3
114157	6	402430	13	NULL	NULL	0	NULL	chromosome 13q	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of heterozygosity on chromosomes 10q , 9p , 17p and 13q in malays with malignant glioma .
	manualset3
114158	7	402430	13	NULL	NULL	0	NULL	malays	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of heterozygosity on chromosomes 10q , 9p , 17p and 13q in malays with malignant glioma .
	manualset3
114159	8	402430	13	NULL	NULL	0	NULL	malignant glioma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of heterozygosity on chromosomes 10q , 9p , 17p and 13q in malays with malignant glioma .
	manualset3
114160	1	402431	13	NULL	NULL	0	NULL	Loss	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of imprinting in human cancer .
	manualset3
114161	2	402431	13	NULL	NULL	0	NULL	human cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of imprinting in human cancer .
	manualset3
119329	3	402431	13	NULL	NULL	0	NULL	imprinting	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss of imprinting in human cancer .
	manualset3
114162	1	402432	13	NULL	NULL	0	NULL	Loss 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss or low expression ( & lt ; 20 % immunoreactive cells ) of LKB1 protein expression was more frequently observed in high-grade NE tumors ( SCLC and LCNEC ; 45/53 , 84.9 % ) than in typical and atypical carcinoids ( 3/15 ; 20 % ) .
	manualset3
114163	2	402432	13	NULL	NULL	0	NULL	low expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss or low expression ( & lt ; 20 % immunoreactive cells ) of LKB1 protein expression was more frequently observed in high-grade NE tumors ( SCLC and LCNEC ; 45/53 , 84.9 % ) than in typical and atypical carcinoids ( 3/15 ; 20 % ) .
	manualset3
114164	3	402432	13	NULL	NULL	0	NULL	20 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss or low expression ( & lt ; 20 % immunoreactive cells ) of LKB1 protein expression was more frequently observed in high-grade NE tumors ( SCLC and LCNEC ; 45/53 , 84.9 % ) than in typical and atypical carcinoids ( 3/15 ; 20 % ) .
	manualset3
114165	4	402432	13	NULL	NULL	0	NULL	immunoreactive cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss or low expression ( & lt ; 20 % immunoreactive cells ) of LKB1 protein expression was more frequently observed in high-grade NE tumors ( SCLC and LCNEC ; 45/53 , 84.9 % ) than in typical and atypical carcinoids ( 3/15 ; 20 % ) .
	manualset3
114166	5	402432	13	NULL	NULL	0	NULL	LKB1 protein expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss or low expression ( & lt ; 20 % immunoreactive cells ) of LKB1 protein expression was more frequently observed in high-grade NE tumors ( SCLC and LCNEC ; 45/53 , 84.9 % ) than in typical and atypical carcinoids ( 3/15 ; 20 % ) .
	manualset3
114167	6	402432	13	NULL	NULL	0	NULL	high-grade NE tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss or low expression ( & lt ; 20 % immunoreactive cells ) of LKB1 protein expression was more frequently observed in high-grade NE tumors ( SCLC and LCNEC ; 45/53 , 84.9 % ) than in typical and atypical carcinoids ( 3/15 ; 20 % ) .
	manualset3
114168	7	402432	13	NULL	NULL	0	NULL	SCLC	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss or low expression ( & lt ; 20 % immunoreactive cells ) of LKB1 protein expression was more frequently observed in high-grade NE tumors ( SCLC and LCNEC ; 45/53 , 84.9 % ) than in typical and atypical carcinoids ( 3/15 ; 20 % ) .
	manualset3
114169	8	402432	13	NULL	NULL	0	NULL	LCNEC 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss or low expression ( & lt ; 20 % immunoreactive cells ) of LKB1 protein expression was more frequently observed in high-grade NE tumors ( SCLC and LCNEC ; 45/53 , 84.9 % ) than in typical and atypical carcinoids ( 3/15 ; 20 % ) .
	manualset3
114170	9	402432	13	NULL	NULL	0	NULL	45/53 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss or low expression ( & lt ; 20 % immunoreactive cells ) of LKB1 protein expression was more frequently observed in high-grade NE tumors ( SCLC and LCNEC ; 45/53 , 84.9 % ) than in typical and atypical carcinoids ( 3/15 ; 20 % ) .
	manualset3
114171	10	402432	13	NULL	NULL	0	NULL	84.9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss or low expression ( & lt ; 20 % immunoreactive cells ) of LKB1 protein expression was more frequently observed in high-grade NE tumors ( SCLC and LCNEC ; 45/53 , 84.9 % ) than in typical and atypical carcinoids ( 3/15 ; 20 % ) .
	manualset3
114172	11	402432	13	NULL	NULL	0	NULL	typical carcinoids	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss or low expression ( & lt ; 20 % immunoreactive cells ) of LKB1 protein expression was more frequently observed in high-grade NE tumors ( SCLC and LCNEC ; 45/53 , 84.9 % ) than in typical and atypical carcinoids ( 3/15 ; 20 % ) .
	manualset3
114173	12	402432	13	NULL	NULL	0	NULL	atypical carcinoids	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss or low expression ( & lt ; 20 % immunoreactive cells ) of LKB1 protein expression was more frequently observed in high-grade NE tumors ( SCLC and LCNEC ; 45/53 , 84.9 % ) than in typical and atypical carcinoids ( 3/15 ; 20 % ) .
	manualset3
114174	13	402432	13	NULL	NULL	0	NULL	3/15	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss or low expression ( & lt ; 20 % immunoreactive cells ) of LKB1 protein expression was more frequently observed in high-grade NE tumors ( SCLC and LCNEC ; 45/53 , 84.9 % ) than in typical and atypical carcinoids ( 3/15 ; 20 % ) .
	manualset3
114175	14	402432	13	NULL	NULL	0	NULL	20 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Loss or low expression ( & lt ; 20 % immunoreactive cells ) of LKB1 protein expression was more frequently observed in high-grade NE tumors ( SCLC and LCNEC ; 45/53 , 84.9 % ) than in typical and atypical carcinoids ( 3/15 ; 20 % ) .
	manualset3
114176	1	402433	13	NULL	NULL	0	NULL	Loudness enhancement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Loudness enhancement and decrement in four paradigms .
	manualset3
114177	2	402433	13	NULL	NULL	0	NULL	decrement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Loudness enhancement and decrement in four paradigms .
	manualset3
114178	3	402433	13	NULL	NULL	0	NULL	four paradigms	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Loudness enhancement and decrement in four paradigms .
	manualset3
114179	1	402434	13	NULL	NULL	0	NULL	Low-density lipoprotein ( LDL ) receptor-related protein-1 ( LRP1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-density lipoprotein ( LDL ) receptor-related protein-1 ( LRP1 ) has been shown to mediate endothelial cell responses to PF4 and so we tested this receptor 's importance in PF4 's role in megakaryopoiesis .
	manualset3
114180	2	402434	13	NULL	NULL	0	NULL	endothelial cell responses 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-density lipoprotein ( LDL ) receptor-related protein-1 ( LRP1 ) has been shown to mediate endothelial cell responses to PF4 and so we tested this receptor 's importance in PF4 's role in megakaryopoiesis .
	manualset3
114181	3	402434	13	NULL	NULL	0	NULL	PF4 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-density lipoprotein ( LDL ) receptor-related protein-1 ( LRP1 ) has been shown to mediate endothelial cell responses to PF4 and so we tested this receptor 's importance in PF4 's role in megakaryopoiesis .
	manualset3
114182	4	402434	13	NULL	NULL	0	NULL	receptor 's	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-density lipoprotein ( LDL ) receptor-related protein-1 ( LRP1 ) has been shown to mediate endothelial cell responses to PF4 and so we tested this receptor 's importance in PF4 's role in megakaryopoiesis .
	manualset3
114183	5	402434	13	NULL	NULL	0	NULL	PF4 's role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-density lipoprotein ( LDL ) receptor-related protein-1 ( LRP1 ) has been shown to mediate endothelial cell responses to PF4 and so we tested this receptor 's importance in PF4 's role in megakaryopoiesis .
	manualset3
114184	6	402434	13	NULL	NULL	0	NULL	megakaryopoiesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-density lipoprotein ( LDL ) receptor-related protein-1 ( LRP1 ) has been shown to mediate endothelial cell responses to PF4 and so we tested this receptor 's importance in PF4 's role in megakaryopoiesis .
	manualset3
114185	1	402435	13	NULL	NULL	0	NULL	Low-digestible carbohydrate 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-digestible carbohydrate fermentation in the gut causes gastrointestinal effects , especially at higher intakes .
	manualset3
114186	2	402435	13	NULL	NULL	0	NULL	fermentation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-digestible carbohydrate fermentation in the gut causes gastrointestinal effects , especially at higher intakes .
	manualset3
114187	3	402435	13	NULL	NULL	0	NULL	gut	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-digestible carbohydrate fermentation in the gut causes gastrointestinal effects , especially at higher intakes .
	manualset3
114188	4	402435	13	NULL	NULL	0	NULL	gastrointestinal effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-digestible carbohydrate fermentation in the gut causes gastrointestinal effects , especially at higher intakes .
	manualset3
114189	5	402435	13	NULL	NULL	0	NULL	causes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-digestible carbohydrate fermentation in the gut causes gastrointestinal effects , especially at higher intakes .
	manualset3
114190	6	402435	13	NULL	NULL	0	NULL	higher intakes	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-digestible carbohydrate fermentation in the gut causes gastrointestinal effects , especially at higher intakes .
	manualset3
114191	1	402436	13	NULL	NULL	0	NULL	Low-energy lasers	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-energy lasers are currently being used in the therapy of rheumatoid arthritis , chronic pain , muscle strain , and the promotion of wound healing in human and veterinary medicine .
	manualset3
114192	2	402436	13	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-energy lasers are currently being used in the therapy of rheumatoid arthritis , chronic pain , muscle strain , and the promotion of wound healing in human and veterinary medicine .
	manualset3
114193	3	402436	13	NULL	NULL	0	NULL	rheumatoid arthritis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-energy lasers are currently being used in the therapy of rheumatoid arthritis , chronic pain , muscle strain , and the promotion of wound healing in human and veterinary medicine .
	manualset3
114194	4	402436	13	NULL	NULL	0	NULL	chronic pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-energy lasers are currently being used in the therapy of rheumatoid arthritis , chronic pain , muscle strain , and the promotion of wound healing in human and veterinary medicine .
	manualset3
114195	5	402436	13	NULL	NULL	0	NULL	muscle strain 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-energy lasers are currently being used in the therapy of rheumatoid arthritis , chronic pain , muscle strain , and the promotion of wound healing in human and veterinary medicine .
	manualset3
114196	6	402436	13	NULL	NULL	0	NULL	promotion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-energy lasers are currently being used in the therapy of rheumatoid arthritis , chronic pain , muscle strain , and the promotion of wound healing in human and veterinary medicine .
	manualset3
114197	7	402436	13	NULL	NULL	0	NULL	wound healing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-energy lasers are currently being used in the therapy of rheumatoid arthritis , chronic pain , muscle strain , and the promotion of wound healing in human and veterinary medicine .
	manualset3
114198	8	402436	13	NULL	NULL	0	NULL	human medicine	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-energy lasers are currently being used in the therapy of rheumatoid arthritis , chronic pain , muscle strain , and the promotion of wound healing in human and veterinary medicine .
	manualset3
114199	9	402436	13	NULL	NULL	0	NULL	veterinary medicine	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-energy lasers are currently being used in the therapy of rheumatoid arthritis , chronic pain , muscle strain , and the promotion of wound healing in human and veterinary medicine .
	manualset3
114200	1	402437	13	NULL	NULL	0	NULL	Low-level laser therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-level laser therapy stimulates mineralization via increased Runx2 expression and ERK phosphorylation in osteoblasts .
	manualset3
114201	2	402437	13	NULL	NULL	0	NULL	mineralization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-level laser therapy stimulates mineralization via increased Runx2 expression and ERK phosphorylation in osteoblasts .
	manualset3
114202	3	402437	13	NULL	NULL	0	NULL	Runx2 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-level laser therapy stimulates mineralization via increased Runx2 expression and ERK phosphorylation in osteoblasts .
	manualset3
114203	4	402437	13	NULL	NULL	0	NULL	ERK phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-level laser therapy stimulates mineralization via increased Runx2 expression and ERK phosphorylation in osteoblasts .
	manualset3
114204	5	402437	13	NULL	NULL	0	NULL	osteoblasts 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-level laser therapy stimulates mineralization via increased Runx2 expression and ERK phosphorylation in osteoblasts .
	manualset3
114205	1	402438	13	NULL	NULL	0	NULL	Low-molecular-weight heparins ( LMWHs ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-molecular-weight heparins ( LMWHs ) have been shown to be effective in the prevention of deep vein thrombosis ( DVT ) after major orthopaedic surgery , such as total hip replacement ( THR ) .
	manualset3
114206	2	402438	13	NULL	NULL	0	NULL	prevention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-molecular-weight heparins ( LMWHs ) have been shown to be effective in the prevention of deep vein thrombosis ( DVT ) after major orthopaedic surgery , such as total hip replacement ( THR ) .
	manualset3
114207	3	402438	13	NULL	NULL	0	NULL	deep vein thrombosis ( DVT )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-molecular-weight heparins ( LMWHs ) have been shown to be effective in the prevention of deep vein thrombosis ( DVT ) after major orthopaedic surgery , such as total hip replacement ( THR ) .
	manualset3
114208	4	402438	13	NULL	NULL	0	NULL	major orthopaedic surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-molecular-weight heparins ( LMWHs ) have been shown to be effective in the prevention of deep vein thrombosis ( DVT ) after major orthopaedic surgery , such as total hip replacement ( THR ) .
	manualset3
114209	5	402438	13	NULL	NULL	0	NULL	total hip replacement ( THR )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Low-molecular-weight heparins ( LMWHs ) have been shown to be effective in the prevention of deep vein thrombosis ( DVT ) after major orthopaedic surgery , such as total hip replacement ( THR ) .
	manualset3
114210	1	402439	13	NULL	NULL	NULL	NULL	Low GABA levels	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Low GABA levels outside of the epileptic focus may facilitate spread of discharges beyond the focus .
	manualset3
114211	2	402439	13	NULL	NULL	0	NULL	epileptic focus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Low GABA levels outside of the epileptic focus may facilitate spread of discharges beyond the focus .
	manualset3
114212	3	402439	13	NULL	NULL	0	NULL	discharges	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Low GABA levels outside of the epileptic focus may facilitate spread of discharges beyond the focus .
	manualset3
114213	4	402439	13	NULL	NULL	NULL	NULL	focus 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Low GABA levels outside of the epileptic focus may facilitate spread of discharges beyond the focus .
	manualset3
114214	1	402440	13	NULL	NULL	0	NULL	Low HRV 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Low HRV is associated with increased risk of all-cause mortality and is a marker for a wide range of diseases .
	manualset3
114215	2	402440	13	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Low HRV is associated with increased risk of all-cause mortality and is a marker for a wide range of diseases .
	manualset3
114216	3	402440	13	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Low HRV is associated with increased risk of all-cause mortality and is a marker for a wide range of diseases .
	manualset3
114217	4	402440	13	NULL	NULL	0	NULL	marker	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Low HRV is associated with increased risk of all-cause mortality and is a marker for a wide range of diseases .
	manualset3
114218	5	402440	13	NULL	NULL	0	NULL	wide range 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Low HRV is associated with increased risk of all-cause mortality and is a marker for a wide range of diseases .
	manualset3
114219	6	402440	13	NULL	NULL	0	NULL	diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Low HRV is associated with increased risk of all-cause mortality and is a marker for a wide range of diseases .
	manualset3
114220	1	402441	13	NULL	NULL	0	NULL	Low back pain ( LBP ) patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Low back pain ( LBP ) patients have poorer postural control compared to healthy controls , and the importance of assessing and addressing balance is a matter of debate .
	manualset3
114221	2	402441	13	NULL	NULL	0	NULL	postural control 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Low back pain ( LBP ) patients have poorer postural control compared to healthy controls , and the importance of assessing and addressing balance is a matter of debate .
	manualset3
114222	3	402441	13	NULL	NULL	0	NULL	healthy controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Low back pain ( LBP ) patients have poorer postural control compared to healthy controls , and the importance of assessing and addressing balance is a matter of debate .
	manualset3
114223	4	402441	13	NULL	NULL	0	NULL	importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Low back pain ( LBP ) patients have poorer postural control compared to healthy controls , and the importance of assessing and addressing balance is a matter of debate .
	manualset3
114224	5	402441	13	NULL	NULL	0	NULL	balance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Low back pain ( LBP ) patients have poorer postural control compared to healthy controls , and the importance of assessing and addressing balance is a matter of debate .
	manualset3
114225	6	402441	13	NULL	NULL	0	NULL	matter of debate	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Low back pain ( LBP ) patients have poorer postural control compared to healthy controls , and the importance of assessing and addressing balance is a matter of debate .
	manualset3
114226	1	402442	13	NULL	NULL	0	NULL	68-year-old man	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A 68-year-old man developed a small pelvic recurrence near the rectal stump 8 months after a Hartmann procedure for rectal cancer .
	manualset3
114227	2	402442	13	NULL	NULL	0	NULL	small pelvic recurrence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 68-year-old man developed a small pelvic recurrence near the rectal stump 8 months after a Hartmann procedure for rectal cancer .
	manualset3
114228	3	402442	13	NULL	NULL	0	NULL	rectal stump	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A 68-year-old man developed a small pelvic recurrence near the rectal stump 8 months after a Hartmann procedure for rectal cancer .
	manualset3
114229	4	402442	13	NULL	NULL	0	NULL	8 months 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	A 68-year-old man developed a small pelvic recurrence near the rectal stump 8 months after a Hartmann procedure for rectal cancer .
	manualset3
114230	5	402442	13	NULL	NULL	0	NULL	Hartmann procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A 68-year-old man developed a small pelvic recurrence near the rectal stump 8 months after a Hartmann procedure for rectal cancer .
	manualset3
114231	6	402442	13	NULL	NULL	0	NULL	rectal cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A 68-year-old man developed a small pelvic recurrence near the rectal stump 8 months after a Hartmann procedure for rectal cancer .
	manualset3
114232	1	402443	13	NULL	NULL	0	NULL	Low concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Low concentrations of cerebrospinal fluid GABA correlate to a reduced response to phenobarbital therapy in primary canine epilepsy .
	manualset3
114233	2	402443	13	NULL	NULL	0	NULL	cerebrospinal fluid GABA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Low concentrations of cerebrospinal fluid GABA correlate to a reduced response to phenobarbital therapy in primary canine epilepsy .
	manualset3
114236	3	402443	13	NULL	NULL	0	NULL	response 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Low concentrations of cerebrospinal fluid GABA correlate to a reduced response to phenobarbital therapy in primary canine epilepsy .
	manualset3
114237	4	402443	13	NULL	NULL	0	NULL	phenobarbital therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Low concentrations of cerebrospinal fluid GABA correlate to a reduced response to phenobarbital therapy in primary canine epilepsy .
	manualset3
114238	5	402443	13	NULL	NULL	0	NULL	primary canine epilepsy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Low concentrations of cerebrospinal fluid GABA correlate to a reduced response to phenobarbital therapy in primary canine epilepsy .
	manualset3
114241	1	402444	13	NULL	NULL	0	NULL	Low concentrations 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Low concentrations of kynurenic acid , however , did not modify ( 3H ) - kainate ( high and low affinity ) or ( 3H ) - AMPA binding to rat brain membranes .
	manualset3
114243	2	402444	13	NULL	NULL	0	NULL	kynurenic acid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Low concentrations of kynurenic acid , however , did not modify ( 3H ) - kainate ( high and low affinity ) or ( 3H ) - AMPA binding to rat brain membranes .
	manualset3
114245	3	402444	13	NULL	NULL	0	NULL	( 3H ) - kainate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Low concentrations of kynurenic acid , however , did not modify ( 3H ) - kainate ( high and low affinity ) or ( 3H ) - AMPA binding to rat brain membranes .
	manualset3
114248	4	402444	13	NULL	NULL	0	NULL	high affinity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Low concentrations of kynurenic acid , however , did not modify ( 3H ) - kainate ( high and low affinity ) or ( 3H ) - AMPA binding to rat brain membranes .
	manualset3
114249	5	402444	13	NULL	NULL	0	NULL	low affinity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Low concentrations of kynurenic acid , however , did not modify ( 3H ) - kainate ( high and low affinity ) or ( 3H ) - AMPA binding to rat brain membranes .
	manualset3
114250	6	402444	13	NULL	NULL	0	NULL	( 3H ) - AMPA binding	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Low concentrations of kynurenic acid , however , did not modify ( 3H ) - kainate ( high and low affinity ) or ( 3H ) - AMPA binding to rat brain membranes .
	manualset3
114251	7	402444	13	NULL	NULL	0	NULL	rat brain membranes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Low concentrations of kynurenic acid , however , did not modify ( 3H ) - kainate ( high and low affinity ) or ( 3H ) - AMPA binding to rat brain membranes .
	manualset3
114253	1	402445	13	NULL	NULL	0	NULL	Low doses	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Low doses of the dopamine agonist ET-495 were administered to nonpsychotic volunteer subjects by slow intravenous infusion , followed by a bolus of 1.5 -- 2.5 mg haloperidol .
	manualset3
114255	2	402445	13	NULL	NULL	NULL	NULL	dopamine agonist ET-495 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Low doses of the dopamine agonist ET-495 were administered to nonpsychotic volunteer subjects by slow intravenous infusion , followed by a bolus of 1.5 -- 2.5 mg haloperidol .
	manualset3
114257	3	402445	13	NULL	NULL	0	NULL	nonpsychotic volunteer subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Low doses of the dopamine agonist ET-495 were administered to nonpsychotic volunteer subjects by slow intravenous infusion , followed by a bolus of 1.5 -- 2.5 mg haloperidol .
	manualset3
114258	4	402445	13	NULL	NULL	0	NULL	slow intravenous infusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Low doses of the dopamine agonist ET-495 were administered to nonpsychotic volunteer subjects by slow intravenous infusion , followed by a bolus of 1.5 -- 2.5 mg haloperidol .
	manualset3
114260	5	402445	13	NULL	NULL	0	NULL	bolus of 1.5 -- 2.5 mg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Low doses of the dopamine agonist ET-495 were administered to nonpsychotic volunteer subjects by slow intravenous infusion , followed by a bolus of 1.5 -- 2.5 mg haloperidol .
	manualset3
114261	6	402445	13	NULL	NULL	0	NULL	haloperidol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Low doses of the dopamine agonist ET-495 were administered to nonpsychotic volunteer subjects by slow intravenous infusion , followed by a bolus of 1.5 -- 2.5 mg haloperidol .
	manualset3
114355	1	402446	13	NULL	NULL	0	NULL	Low literacy levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Low literacy levels in adults : implications for patient education .
	manualset3
114356	2	402446	13	NULL	NULL	0	NULL	adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Low literacy levels in adults : implications for patient education .
	manualset3
114357	3	402446	13	NULL	NULL	0	NULL	implications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Low literacy levels in adults : implications for patient education .
	manualset3
114358	4	402446	13	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Low literacy levels in adults : implications for patient education .
	manualset3
114359	5	402446	13	NULL	NULL	0	NULL	education 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Low literacy levels in adults : implications for patient education .
	manualset3
114360	1	402447	13	NULL	NULL	0	NULL	Low molecular weight IgM	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Low molecular weight IgM , the monomeric subunit of pentameric IgM , was clearly detected by immunoblotting and filtration chromatographic techniques in six patients with juvenile chronic arthritis and in trace quantities in a further eight of 24 patients studied .
	manualset3
114361	2	402447	13	NULL	NULL	0	NULL	monomeric subunit of pentameric IgM 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Low molecular weight IgM , the monomeric subunit of pentameric IgM , was clearly detected by immunoblotting and filtration chromatographic techniques in six patients with juvenile chronic arthritis and in trace quantities in a further eight of 24 patients studied .
	manualset3
114362	3	402447	13	NULL	NULL	0	NULL	immunoblotting 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Low molecular weight IgM , the monomeric subunit of pentameric IgM , was clearly detected by immunoblotting and filtration chromatographic techniques in six patients with juvenile chronic arthritis and in trace quantities in a further eight of 24 patients studied .
	manualset3
114363	4	402447	13	NULL	NULL	0	NULL	filtration chromatographic techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Low molecular weight IgM , the monomeric subunit of pentameric IgM , was clearly detected by immunoblotting and filtration chromatographic techniques in six patients with juvenile chronic arthritis and in trace quantities in a further eight of 24 patients studied .
	manualset3
114364	5	402447	13	NULL	NULL	0	NULL	six patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Low molecular weight IgM , the monomeric subunit of pentameric IgM , was clearly detected by immunoblotting and filtration chromatographic techniques in six patients with juvenile chronic arthritis and in trace quantities in a further eight of 24 patients studied .
	manualset3
114365	6	402447	13	NULL	NULL	0	NULL	juvenile chronic arthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Low molecular weight IgM , the monomeric subunit of pentameric IgM , was clearly detected by immunoblotting and filtration chromatographic techniques in six patients with juvenile chronic arthritis and in trace quantities in a further eight of 24 patients studied .
	manualset3
114366	7	402447	13	NULL	NULL	0	NULL	trace quantities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Low molecular weight IgM , the monomeric subunit of pentameric IgM , was clearly detected by immunoblotting and filtration chromatographic techniques in six patients with juvenile chronic arthritis and in trace quantities in a further eight of 24 patients studied .
	manualset3
114367	8	402447	13	NULL	NULL	0	NULL	eight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Low molecular weight IgM , the monomeric subunit of pentameric IgM , was clearly detected by immunoblotting and filtration chromatographic techniques in six patients with juvenile chronic arthritis and in trace quantities in a further eight of 24 patients studied .
	manualset3
114368	9	402447	13	NULL	NULL	0	NULL	24 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Low molecular weight IgM , the monomeric subunit of pentameric IgM , was clearly detected by immunoblotting and filtration chromatographic techniques in six patients with juvenile chronic arthritis and in trace quantities in a further eight of 24 patients studied .
	manualset3
114369	1	402448	13	NULL	NULL	0	NULL	Low pH-induced collapse	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Low pH-induced collapse of liposomes containing acid-labile BD2 into micelles was more facile than that of BD1 .
	manualset3
114370	2	402448	13	NULL	NULL	0	NULL	liposomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Low pH-induced collapse of liposomes containing acid-labile BD2 into micelles was more facile than that of BD1 .
	manualset3
114371	3	402448	13	NULL	NULL	0	NULL	acid-labile BD2 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Low pH-induced collapse of liposomes containing acid-labile BD2 into micelles was more facile than that of BD1 .
	manualset3
114372	4	402448	13	NULL	NULL	0	NULL	micelles	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Low pH-induced collapse of liposomes containing acid-labile BD2 into micelles was more facile than that of BD1 .
	manualset3
114373	5	402448	13	NULL	NULL	0	NULL	BD1	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Low pH-induced collapse of liposomes containing acid-labile BD2 into micelles was more facile than that of BD1 .
	manualset3
114374	1	402449	13	NULL	NULL	0	NULL	Low serum mannose-binding protein ( MBP ) concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Low serum mannose-binding protein ( MBP ) concentrations are associated with a common opsonic defect .
	manualset3
114375	2	402449	13	NULL	NULL	0	NULL	opsonic defect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Low serum mannose-binding protein ( MBP ) concentrations are associated with a common opsonic defect .
	manualset3
114376	1	402450	13	NULL	NULL	0	NULL	Low to moderate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Low to moderate Gn concentrations ( 75-75 00 mIUmL ( -1 ) ) effectively improved nuclear maturation and in vitro development .
	manualset3
114377	2	402450	13	NULL	NULL	0	NULL	Gn concentrations 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Low to moderate Gn concentrations ( 75-75 00 mIUmL ( -1 ) ) effectively improved nuclear maturation and in vitro development .
	manualset3
114378	3	402450	13	NULL	NULL	0	NULL	75-75 00 mIUmL ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Low to moderate Gn concentrations ( 75-75 00 mIUmL ( -1 ) ) effectively improved nuclear maturation and in vitro development .
	manualset3
114379	4	402450	13	NULL	NULL	0	NULL	nuclear maturation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Low to moderate Gn concentrations ( 75-75 00 mIUmL ( -1 ) ) effectively improved nuclear maturation and in vitro development .
	manualset3
114380	5	402450	13	NULL	NULL	0	NULL	development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Low to moderate Gn concentrations ( 75-75 00 mIUmL ( -1 ) ) effectively improved nuclear maturation and in vitro development .
	manualset3
114381	1	402451	13	NULL	NULL	0	NULL	7-year-old girl	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A 7-year-old girl presented with a Gartland grade III supracondylar fracture and no radial pulse .
	manualset3
114382	2	402451	13	NULL	NULL	0	NULL	Gartland grade III supracondylar fracture 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 7-year-old girl presented with a Gartland grade III supracondylar fracture and no radial pulse .
	manualset3
114383	3	402451	13	NULL	NULL	0	NULL	radial pulse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 7-year-old girl presented with a Gartland grade III supracondylar fracture and no radial pulse .
	manualset3
114384	1	402452	13	NULL	NULL	0	NULL	Lower third molar 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Lower third molar development in relation to skeletal maturity and chronological age .
	manualset3
114385	2	402452	13	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lower third molar development in relation to skeletal maturity and chronological age .
	manualset3
114386	3	402452	13	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Lower third molar development in relation to skeletal maturity and chronological age .
	manualset3
114387	4	402452	13	NULL	NULL	0	NULL	skeletal maturity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lower third molar development in relation to skeletal maturity and chronological age .
	manualset3
114388	5	402452	13	NULL	NULL	0	NULL	chronological age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Lower third molar development in relation to skeletal maturity and chronological age .
	manualset3
114389	1	402453	13	NULL	NULL	0	NULL	Lowest incidence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lowest incidence of maternal mortality , perinatal mortality , and prematurity occurs in women between 20 and 30 .
	manualset3
114390	2	402453	13	NULL	NULL	0	NULL	maternal mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lowest incidence of maternal mortality , perinatal mortality , and prematurity occurs in women between 20 and 30 .
	manualset3
114391	3	402453	13	NULL	NULL	0	NULL	perinatal mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lowest incidence of maternal mortality , perinatal mortality , and prematurity occurs in women between 20 and 30 .
	manualset3
114392	4	402453	13	NULL	NULL	0	NULL	prematurity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lowest incidence of maternal mortality , perinatal mortality , and prematurity occurs in women between 20 and 30 .
	manualset3
114393	5	402453	13	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Lowest incidence of maternal mortality , perinatal mortality , and prematurity occurs in women between 20 and 30 .
	manualset3
114395	6	402453	13	NULL	NULL	0	NULL	between 20 and 30 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Lowest incidence of maternal mortality , perinatal mortality , and prematurity occurs in women between 20 and 30 .
	manualset3
114402	1	402454	13	NULL	NULL	0	NULL	Loxiglumide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Loxiglumide also decreased contractile frequency during the fed state from 9.7 + / - 0.6 to 8.3 + / - 0.5 / min and reduced the area under contractions to 78 + / - 6 % of the control without loxiglumide ( P less than 0.05 ) .
	manualset3
114403	2	402454	13	NULL	NULL	0	NULL	contractile frequency	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Loxiglumide also decreased contractile frequency during the fed state from 9.7 + / - 0.6 to 8.3 + / - 0.5 / min and reduced the area under contractions to 78 + / - 6 % of the control without loxiglumide ( P less than 0.05 ) .
	manualset3
114405	3	402454	13	NULL	NULL	0	NULL	state	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Loxiglumide also decreased contractile frequency during the fed state from 9.7 + / - 0.6 to 8.3 + / - 0.5 / min and reduced the area under contractions to 78 + / - 6 % of the control without loxiglumide ( P less than 0.05 ) .
	manualset3
114406	4	402454	13	NULL	NULL	0	NULL	9.7 + / - 0.6 to 8.3 + / - 0.5 / min	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Loxiglumide also decreased contractile frequency during the fed state from 9.7 + / - 0.6 to 8.3 + / - 0.5 / min and reduced the area under contractions to 78 + / - 6 % of the control without loxiglumide ( P less than 0.05 ) .
	manualset3
114407	5	402454	13	NULL	NULL	0	NULL	area	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Loxiglumide also decreased contractile frequency during the fed state from 9.7 + / - 0.6 to 8.3 + / - 0.5 / min and reduced the area under contractions to 78 + / - 6 % of the control without loxiglumide ( P less than 0.05 ) .
	manualset3
114408	6	402454	13	NULL	NULL	0	NULL	contractions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Loxiglumide also decreased contractile frequency during the fed state from 9.7 + / - 0.6 to 8.3 + / - 0.5 / min and reduced the area under contractions to 78 + / - 6 % of the control without loxiglumide ( P less than 0.05 ) .
	manualset3
114410	7	402454	13	NULL	NULL	0	NULL	78 + / - 6 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Loxiglumide also decreased contractile frequency during the fed state from 9.7 + / - 0.6 to 8.3 + / - 0.5 / min and reduced the area under contractions to 78 + / - 6 % of the control without loxiglumide ( P less than 0.05 ) .
	manualset3
114412	8	402454	13	NULL	NULL	0	NULL	control 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Loxiglumide also decreased contractile frequency during the fed state from 9.7 + / - 0.6 to 8.3 + / - 0.5 / min and reduced the area under contractions to 78 + / - 6 % of the control without loxiglumide ( P less than 0.05 ) .
	manualset3
114414	9	402454	13	NULL	NULL	0	NULL	loxiglumide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Loxiglumide also decreased contractile frequency during the fed state from 9.7 + / - 0.6 to 8.3 + / - 0.5 / min and reduced the area under contractions to 78 + / - 6 % of the control without loxiglumide ( P less than 0.05 ) .
	manualset3
114415	10	402454	13	NULL	NULL	0	NULL	P less than 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Loxiglumide also decreased contractile frequency during the fed state from 9.7 + / - 0.6 to 8.3 + / - 0.5 / min and reduced the area under contractions to 78 + / - 6 % of the control without loxiglumide ( P less than 0.05 ) .
	manualset3
114418	1	402455	13	NULL	NULL	0	NULL	Japan	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Ltd. , Japan ) for the identification of methicillin-resistant Staphylococcus aureus was evaluated in comparison with the BBL Crystal MRSA ID System ( Becton Dickinson Europe , France ) .
	manualset3
114420	2	402455	13	NULL	NULL	0	NULL	identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ltd. , Japan ) for the identification of methicillin-resistant Staphylococcus aureus was evaluated in comparison with the BBL Crystal MRSA ID System ( Becton Dickinson Europe , France ) .
	manualset3
114421	3	402455	13	NULL	NULL	0	NULL	methicillin-resistant Staphylococcus aureus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ltd. , Japan ) for the identification of methicillin-resistant Staphylococcus aureus was evaluated in comparison with the BBL Crystal MRSA ID System ( Becton Dickinson Europe , France ) .
	manualset3
114422	4	402455	13	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Ltd. , Japan ) for the identification of methicillin-resistant Staphylococcus aureus was evaluated in comparison with the BBL Crystal MRSA ID System ( Becton Dickinson Europe , France ) .
	manualset3
114423	5	402455	13	NULL	NULL	0	NULL	BBL Crystal MRSA ID System	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ltd. , Japan ) for the identification of methicillin-resistant Staphylococcus aureus was evaluated in comparison with the BBL Crystal MRSA ID System ( Becton Dickinson Europe , France ) .
	manualset3
114424	6	402455	13	NULL	NULL	0	NULL	Becton Dickinson Europe	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Ltd. , Japan ) for the identification of methicillin-resistant Staphylococcus aureus was evaluated in comparison with the BBL Crystal MRSA ID System ( Becton Dickinson Europe , France ) .
	manualset3
114425	7	402455	13	NULL	NULL	0	NULL	France	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Ltd. , Japan ) for the identification of methicillin-resistant Staphylococcus aureus was evaluated in comparison with the BBL Crystal MRSA ID System ( Becton Dickinson Europe , France ) .
	manualset3
114481	1	402456	13	NULL	NULL	0	NULL	Luminal flow 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Luminal flow stimulates NO production by nitric oxide synthase type 3 and its translocation to the apical membrane in medullary thick ascending limbs .
	manualset3
114482	2	402456	13	NULL	NULL	0	NULL	NO production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Luminal flow stimulates NO production by nitric oxide synthase type 3 and its translocation to the apical membrane in medullary thick ascending limbs .
	manualset3
114483	3	402456	13	NULL	NULL	0	NULL	nitric oxide synthase type 3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Luminal flow stimulates NO production by nitric oxide synthase type 3 and its translocation to the apical membrane in medullary thick ascending limbs .
	manualset3
114484	4	402456	13	NULL	NULL	0	NULL	translocation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Luminal flow stimulates NO production by nitric oxide synthase type 3 and its translocation to the apical membrane in medullary thick ascending limbs .
	manualset3
114485	5	402456	13	NULL	NULL	0	NULL	apical membrane	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Luminal flow stimulates NO production by nitric oxide synthase type 3 and its translocation to the apical membrane in medullary thick ascending limbs .
	manualset3
114486	6	402456	13	NULL	NULL	0	NULL	medullary thick ascending limbs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Luminal flow stimulates NO production by nitric oxide synthase type 3 and its translocation to the apical membrane in medullary thick ascending limbs .
	manualset3
114487	1	402457	13	NULL	NULL	0	NULL	Lung abscess	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lung abscess was diagnosed during a complex examination in 115 patients .
	manualset3
114488	2	402457	13	NULL	NULL	0	NULL	complex examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Lung abscess was diagnosed during a complex examination in 115 patients .
	manualset3
114489	3	402457	13	NULL	NULL	0	NULL	115 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Lung abscess was diagnosed during a complex examination in 115 patients .
	manualset3
114490	1	402458	13	NULL	NULL	0	NULL	Lung cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Lung cancer , breast cancer , and melanoma are the most frequent to develop brain metastases , and account for 67 % -80 % of all cancers .
	manualset3
114491	2	402458	13	NULL	NULL	0	NULL	breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Lung cancer , breast cancer , and melanoma are the most frequent to develop brain metastases , and account for 67 % -80 % of all cancers .
	manualset3
114492	3	402458	13	NULL	NULL	0	NULL	melanoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Lung cancer , breast cancer , and melanoma are the most frequent to develop brain metastases , and account for 67 % -80 % of all cancers .
	manualset3
114493	4	402458	13	NULL	NULL	0	NULL	brain metastases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lung cancer , breast cancer , and melanoma are the most frequent to develop brain metastases , and account for 67 % -80 % of all cancers .
	manualset3
114494	5	402458	13	NULL	NULL	0	NULL	account	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Lung cancer , breast cancer , and melanoma are the most frequent to develop brain metastases , and account for 67 % -80 % of all cancers .
	manualset3
114495	6	402458	13	NULL	NULL	0	NULL	 67 % -80 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Lung cancer , breast cancer , and melanoma are the most frequent to develop brain metastases , and account for 67 % -80 % of all cancers .
	manualset3
114496	7	402458	13	NULL	NULL	0	NULL	cancers 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Lung cancer , breast cancer , and melanoma are the most frequent to develop brain metastases , and account for 67 % -80 % of all cancers .
	manualset3
114497	1	402459	13	NULL	NULL	0	NULL	Lung cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Lung cancer , cervical cancer , colon cancer and prostate cancer are among the top 10 cancer types worldwide .
	manualset3
114498	2	402459	13	NULL	NULL	0	NULL	cervical cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Lung cancer , cervical cancer , colon cancer and prostate cancer are among the top 10 cancer types worldwide .
	manualset3
114499	3	402459	13	NULL	NULL	0	NULL	colon cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Lung cancer , cervical cancer , colon cancer and prostate cancer are among the top 10 cancer types worldwide .
	manualset3
114500	4	402459	13	NULL	NULL	0	NULL	prostate cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Lung cancer , cervical cancer , colon cancer and prostate cancer are among the top 10 cancer types worldwide .
	manualset3
114501	5	402459	13	NULL	NULL	0	NULL	top 10 cancer types	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lung cancer , cervical cancer , colon cancer and prostate cancer are among the top 10 cancer types worldwide .
	manualset3
114502	1	402460	13	NULL	NULL	0	NULL	Lung cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Lung cancer is the leading cause of cancer-related death in men and the second leading cause in women .
	manualset3
114503	2	402460	13	NULL	NULL	0	NULL	cause 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lung cancer is the leading cause of cancer-related death in men and the second leading cause in women .
	manualset3
114504	3	402460	13	NULL	NULL	0	NULL	cancer-related death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lung cancer is the leading cause of cancer-related death in men and the second leading cause in women .
	manualset3
114505	4	402460	13	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Lung cancer is the leading cause of cancer-related death in men and the second leading cause in women .
	manualset3
114506	5	402460	13	NULL	NULL	0	NULL	cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lung cancer is the leading cause of cancer-related death in men and the second leading cause in women .
	manualset3
114507	6	402460	13	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Lung cancer is the leading cause of cancer-related death in men and the second leading cause in women .
	manualset3
114508	1	402461	13	NULL	NULL	0	NULL	7-year-old girl	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A 7-year-old girl presented with pain and progressive swelling on the left plantar surface .
	manualset3
114509	2	402461	13	NULL	NULL	0	NULL	pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 7-year-old girl presented with pain and progressive swelling on the left plantar surface .
	manualset3
114510	3	402461	13	NULL	NULL	0	NULL	progressive swelling	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 7-year-old girl presented with pain and progressive swelling on the left plantar surface .
	manualset3
114511	4	402461	13	NULL	NULL	0	NULL	left plantar surface	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 7-year-old girl presented with pain and progressive swelling on the left plantar surface .
	manualset3
114512	1	402462	13	NULL	NULL	0	NULL	Lung function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lung function and symptom perception in children with asthma and their parents .
	manualset3
114513	2	402462	13	NULL	NULL	0	NULL	symptom perception 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lung function and symptom perception in children with asthma and their parents .
	manualset3
114514	3	402462	13	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Lung function and symptom perception in children with asthma and their parents .
	manualset3
114515	4	402462	13	NULL	NULL	0	NULL	asthma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lung function and symptom perception in children with asthma and their parents .
	manualset3
114516	5	402462	13	NULL	NULL	0	NULL	parents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Lung function and symptom perception in children with asthma and their parents .
	manualset3
114517	1	402463	13	NULL	NULL	0	NULL	Lung perfusion scintigraphy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Lung perfusion scintigraphy with technetium-labeled macroaggregated albumin was performed on the fourth day after the operation .
	manualset3
114518	2	402463	13	NULL	NULL	NULL	NULL	albumin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Lung perfusion scintigraphy with technetium-labeled macroaggregated albumin was performed on the fourth day after the operation .
	manualset3
114519	3	402463	13	NULL	NULL	0	NULL	fourth day	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Lung perfusion scintigraphy with technetium-labeled macroaggregated albumin was performed on the fourth day after the operation .
	manualset3
114520	4	402463	13	NULL	NULL	0	NULL	operation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Lung perfusion scintigraphy with technetium-labeled macroaggregated albumin was performed on the fourth day after the operation .
	manualset3
114614	1	402464	13	NULL	NULL	0	NULL	Luteal phase estradiol level 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Luteal phase estradiol level : a potential predictive marker for successful pregnancy in in vitro fertilization/intracytoplasmic sperm injection .
	manualset3
114615	2	402464	13	NULL	NULL	0	NULL	predictive marker	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Luteal phase estradiol level : a potential predictive marker for successful pregnancy in in vitro fertilization/intracytoplasmic sperm injection .
	manualset3
114616	3	402464	13	NULL	NULL	0	NULL	successful pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Luteal phase estradiol level : a potential predictive marker for successful pregnancy in in vitro fertilization/intracytoplasmic sperm injection .
	manualset3
114617	4	402464	13	NULL	NULL	0	NULL	in vitro fertilization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Luteal phase estradiol level : a potential predictive marker for successful pregnancy in in vitro fertilization/intracytoplasmic sperm injection .
	manualset3
114618	5	402464	13	NULL	NULL	0	NULL	intracytoplasmic sperm injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Luteal phase estradiol level : a potential predictive marker for successful pregnancy in in vitro fertilization/intracytoplasmic sperm injection .
	manualset3
114619	1	402465	13	NULL	NULL	0	NULL	Luteinizing hormone-releasing hormone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Luteinizing hormone-releasing hormone and gamma-aminobutyric acid neurons in the medial preoptic area are synaptic targets of dopamine axons originating in anterior periventricular areas .
	manualset3
114676	2	402465	13	NULL	NULL	0	NULL	gamma-aminobutyric acid neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Luteinizing hormone-releasing hormone and gamma-aminobutyric acid neurons in the medial preoptic area are synaptic targets of dopamine axons originating in anterior periventricular areas .
	manualset3
114677	3	402465	13	NULL	NULL	0	NULL	medial preoptic area	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Luteinizing hormone-releasing hormone and gamma-aminobutyric acid neurons in the medial preoptic area are synaptic targets of dopamine axons originating in anterior periventricular areas .
	manualset3
114678	4	402465	13	NULL	NULL	0	NULL	synaptic targets	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Luteinizing hormone-releasing hormone and gamma-aminobutyric acid neurons in the medial preoptic area are synaptic targets of dopamine axons originating in anterior periventricular areas .
	manualset3
114679	5	402465	13	NULL	NULL	0	NULL	dopamine axons	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Luteinizing hormone-releasing hormone and gamma-aminobutyric acid neurons in the medial preoptic area are synaptic targets of dopamine axons originating in anterior periventricular areas .
	manualset3
114680	6	402465	13	NULL	NULL	0	NULL	anterior periventricular areas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Luteinizing hormone-releasing hormone and gamma-aminobutyric acid neurons in the medial preoptic area are synaptic targets of dopamine axons originating in anterior periventricular areas .
	manualset3
114681	1	402466	13	NULL	NULL	NULL	NULL	LvDcr1 expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	LvDcr1 expression regularly increased at the upper phase of nauplius , zoea and mysis stages than their prophase .
	manualset3
114682	2	402466	13	NULL	NULL	NULL	NULL	upper phase	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	LvDcr1 expression regularly increased at the upper phase of nauplius , zoea and mysis stages than their prophase .
	manualset3
114683	3	402466	13	NULL	NULL	0	NULL	nauplius stage	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	LvDcr1 expression regularly increased at the upper phase of nauplius , zoea and mysis stages than their prophase .
	manualset3
114684	4	402466	13	NULL	NULL	0	NULL	zoea stage	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	LvDcr1 expression regularly increased at the upper phase of nauplius , zoea and mysis stages than their prophase .
	manualset3
114685	5	402466	13	NULL	NULL	0	NULL	mysis stage	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	LvDcr1 expression regularly increased at the upper phase of nauplius , zoea and mysis stages than their prophase .
	manualset3
114686	6	402466	13	NULL	NULL	0	NULL	prophase 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	LvDcr1 expression regularly increased at the upper phase of nauplius , zoea and mysis stages than their prophase .
	manualset3
114687	1	402467	13	NULL	NULL	0	NULL	Lycopene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lycopene and apigenin were observed to block the endothelial cell proliferation in a dose-dependent manner .
	manualset3
114688	2	402467	13	NULL	NULL	0	NULL	apigenin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lycopene and apigenin were observed to block the endothelial cell proliferation in a dose-dependent manner .
	manualset3
114689	3	402467	13	NULL	NULL	0	NULL	endothelial cell 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Lycopene and apigenin were observed to block the endothelial cell proliferation in a dose-dependent manner .
	manualset3
114690	4	402467	13	NULL	NULL	0	NULL	 proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lycopene and apigenin were observed to block the endothelial cell proliferation in a dose-dependent manner .
	manualset3
114691	5	402467	13	NULL	NULL	0	NULL	dose-dependent manner	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Lycopene and apigenin were observed to block the endothelial cell proliferation in a dose-dependent manner .
	manualset3
114692	1	402468	13	NULL	NULL	0	NULL	Lymph drainage 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymph drainage of the human uterus .
	manualset3
114693	2	402468	13	NULL	NULL	0	NULL	human uterus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymph drainage of the human uterus .
	manualset3
114694	1	402469	13	NULL	NULL	0	NULL	Lymph node biopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymph node biopsy suggested splenic marginal zone B-cell lymphoma .
	manualset3
114695	2	402469	13	NULL	NULL	0	NULL	splenic marginal zone B-cell lymphoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymph node biopsy suggested splenic marginal zone B-cell lymphoma .
	manualset3
114696	1	402470	13	NULL	NULL	0	NULL	71-year-old woman	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A 71-year-old woman was admitted in December 2002 because of lymphadenopathy , hepatosplenomegaly and pleural effusion .
	manualset3
114697	2	402470	13	NULL	NULL	0	NULL	December 2002	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	A 71-year-old woman was admitted in December 2002 because of lymphadenopathy , hepatosplenomegaly and pleural effusion .
	manualset3
114698	3	402470	13	NULL	NULL	0	NULL	lymphadenopathy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 71-year-old woman was admitted in December 2002 because of lymphadenopathy , hepatosplenomegaly and pleural effusion .
	manualset3
114699	4	402470	13	NULL	NULL	0	NULL	hepatosplenomegaly 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 71-year-old woman was admitted in December 2002 because of lymphadenopathy , hepatosplenomegaly and pleural effusion .
	manualset3
114700	5	402470	13	NULL	NULL	0	NULL	pleural effusion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 71-year-old woman was admitted in December 2002 because of lymphadenopathy , hepatosplenomegaly and pleural effusion .
	manualset3
114701	1	402471	13	NULL	NULL	0	NULL	Lymph node counts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymph node counts in 58 patients who received preoperative neoadjuvant chemotherapy were compared with those in 168 patients who received surgery alone .
	manualset3
114702	2	402471	13	NULL	NULL	0	NULL	58 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymph node counts in 58 patients who received preoperative neoadjuvant chemotherapy were compared with those in 168 patients who received surgery alone .
	manualset3
114703	3	402471	13	NULL	NULL	0	NULL	preoperative neoadjuvant chemotherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymph node counts in 58 patients who received preoperative neoadjuvant chemotherapy were compared with those in 168 patients who received surgery alone .
	manualset3
114704	4	402471	13	NULL	NULL	0	NULL	168 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymph node counts in 58 patients who received preoperative neoadjuvant chemotherapy were compared with those in 168 patients who received surgery alone .
	manualset3
114705	5	402471	13	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymph node counts in 58 patients who received preoperative neoadjuvant chemotherapy were compared with those in 168 patients who received surgery alone .
	manualset3
114706	1	402472	13	NULL	NULL	0	NULL	Lymph nodes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymph nodes other than regional showed no CI response at any time in either tumor system .
	manualset3
114707	2	402472	13	NULL	NULL	0	NULL	CI response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymph nodes other than regional showed no CI response at any time in either tumor system .
	manualset3
114708	3	402472	13	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymph nodes other than regional showed no CI response at any time in either tumor system .
	manualset3
114709	4	402472	13	NULL	NULL	0	NULL	tumor system	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymph nodes other than regional showed no CI response at any time in either tumor system .
	manualset3
114710	1	402473	13	NULL	NULL	0	NULL	Lymphangioma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphangioma are uncommon hamartomatous congenital malformations of the lymphatic system that involve skin and subcutaneous tissue .
	manualset3
114711	2	402473	13	NULL	NULL	0	NULL	congenital malformations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphangioma are uncommon hamartomatous congenital malformations of the lymphatic system that involve skin and subcutaneous tissue .
	manualset3
114712	3	402473	13	NULL	NULL	0	NULL	lymphatic system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphangioma are uncommon hamartomatous congenital malformations of the lymphatic system that involve skin and subcutaneous tissue .
	manualset3
114713	4	402473	13	NULL	NULL	0	NULL	skin 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphangioma are uncommon hamartomatous congenital malformations of the lymphatic system that involve skin and subcutaneous tissue .
	manualset3
114714	5	402473	13	NULL	NULL	0	NULL	subcutaneous tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphangioma are uncommon hamartomatous congenital malformations of the lymphatic system that involve skin and subcutaneous tissue .
	manualset3
114715	1	402474	13	NULL	NULL	0	NULL	Lymphangioma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphangioma of the lesser omentum associated with abdominal esophageal carcinoma : report of a case .
	manualset3
114716	2	402474	13	NULL	NULL	0	NULL	omentum 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphangioma of the lesser omentum associated with abdominal esophageal carcinoma : report of a case .
	manualset3
114717	3	402474	13	NULL	NULL	0	NULL	abdominal esophageal carcinoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphangioma of the lesser omentum associated with abdominal esophageal carcinoma : report of a case .
	manualset3
114718	4	402474	13	NULL	NULL	0	NULL	report 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphangioma of the lesser omentum associated with abdominal esophageal carcinoma : report of a case .
	manualset3
114719	5	402474	13	NULL	NULL	0	NULL	case	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphangioma of the lesser omentum associated with abdominal esophageal carcinoma : report of a case .
	manualset3
114720	1	402475	13	NULL	NULL	0	NULL	Lymphocyte subpopulations 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocyte subpopulations and mitogenic responses in nasopharyngeal carcinoma , prior to and after radiotherapy .
	manualset3
114721	2	402475	13	NULL	NULL	0	NULL	mitogenic responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocyte subpopulations and mitogenic responses in nasopharyngeal carcinoma , prior to and after radiotherapy .
	manualset3
114722	3	402475	13	NULL	NULL	0	NULL	nasopharyngeal carcinoma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocyte subpopulations and mitogenic responses in nasopharyngeal carcinoma , prior to and after radiotherapy .
	manualset3
114723	4	402475	13	NULL	NULL	0	NULL	radiotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocyte subpopulations and mitogenic responses in nasopharyngeal carcinoma , prior to and after radiotherapy .
	manualset3
114726	1	402476	13	NULL	NULL	0	NULL	Lymphocyte surface antigen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocyte surface antigen CD3 , CD4 , CD8 , HLA-DR and CD25 were stained in appropriate combination and detected with fluorescence-activated cell sorter analysis .
	manualset3
114730	2	402476	13	NULL	NULL	0	NULL	CD3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocyte surface antigen CD3 , CD4 , CD8 , HLA-DR and CD25 were stained in appropriate combination and detected with fluorescence-activated cell sorter analysis .
	manualset3
114731	3	402476	13	NULL	NULL	0	NULL	CD4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocyte surface antigen CD3 , CD4 , CD8 , HLA-DR and CD25 were stained in appropriate combination and detected with fluorescence-activated cell sorter analysis .
	manualset3
114732	4	402476	13	NULL	NULL	0	NULL	CD8	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocyte surface antigen CD3 , CD4 , CD8 , HLA-DR and CD25 were stained in appropriate combination and detected with fluorescence-activated cell sorter analysis .
	manualset3
114733	5	402476	13	NULL	NULL	0	NULL	HLA-DR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocyte surface antigen CD3 , CD4 , CD8 , HLA-DR and CD25 were stained in appropriate combination and detected with fluorescence-activated cell sorter analysis .
	manualset3
114734	6	402476	13	NULL	NULL	0	NULL	CD25	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocyte surface antigen CD3 , CD4 , CD8 , HLA-DR and CD25 were stained in appropriate combination and detected with fluorescence-activated cell sorter analysis .
	manualset3
114735	7	402476	13	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocyte surface antigen CD3 , CD4 , CD8 , HLA-DR and CD25 were stained in appropriate combination and detected with fluorescence-activated cell sorter analysis .
	manualset3
114736	8	402476	13	NULL	NULL	0	NULL	fluorescence-activated cell sorter analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocyte surface antigen CD3 , CD4 , CD8 , HLA-DR and CD25 were stained in appropriate combination and detected with fluorescence-activated cell sorter analysis .
	manualset3
114739	1	402477	13	NULL	NULL	0	NULL	Lymphocyte transformation tests	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocyte transformation tests performed on lymph node cells of mice infected or immunized with leprosy bacilli also showed the leprosy bacillus to have a closer relationship with M. vaccae than with other mycobacteria .
	manualset3
114740	2	402477	13	NULL	NULL	0	NULL	lymph node cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocyte transformation tests performed on lymph node cells of mice infected or immunized with leprosy bacilli also showed the leprosy bacillus to have a closer relationship with M. vaccae than with other mycobacteria .
	manualset3
114742	3	402477	13	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocyte transformation tests performed on lymph node cells of mice infected or immunized with leprosy bacilli also showed the leprosy bacillus to have a closer relationship with M. vaccae than with other mycobacteria .
	manualset3
114744	4	402477	13	NULL	NULL	0	NULL	leprosy bacilli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocyte transformation tests performed on lymph node cells of mice infected or immunized with leprosy bacilli also showed the leprosy bacillus to have a closer relationship with M. vaccae than with other mycobacteria .
	manualset3
114745	5	402477	13	NULL	NULL	0	NULL	leprosy bacillus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocyte transformation tests performed on lymph node cells of mice infected or immunized with leprosy bacilli also showed the leprosy bacillus to have a closer relationship with M. vaccae than with other mycobacteria .
	manualset3
114746	6	402477	13	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocyte transformation tests performed on lymph node cells of mice infected or immunized with leprosy bacilli also showed the leprosy bacillus to have a closer relationship with M. vaccae than with other mycobacteria .
	manualset3
114747	7	402477	13	NULL	NULL	0	NULL	M. vaccae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocyte transformation tests performed on lymph node cells of mice infected or immunized with leprosy bacilli also showed the leprosy bacillus to have a closer relationship with M. vaccae than with other mycobacteria .
	manualset3
114749	8	402477	13	NULL	NULL	0	NULL	mycobacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocyte transformation tests performed on lymph node cells of mice infected or immunized with leprosy bacilli also showed the leprosy bacillus to have a closer relationship with M. vaccae than with other mycobacteria .
	manualset3
114752	1	402478	13	NULL	NULL	0	NULL	Lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocytes from ten patients without and one with hypogammaglobulinemia were capable of differentiating into lg-producing cells .
	manualset3
114753	2	402478	13	NULL	NULL	0	NULL	ten patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocytes from ten patients without and one with hypogammaglobulinemia were capable of differentiating into lg-producing cells .
	manualset3
114754	3	402478	13	NULL	NULL	0	NULL	hypogammaglobulinemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocytes from ten patients without and one with hypogammaglobulinemia were capable of differentiating into lg-producing cells .
	manualset3
114755	4	402478	13	NULL	NULL	0	NULL	lg-producing cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocytes from ten patients without and one with hypogammaglobulinemia were capable of differentiating into lg-producing cells .
	manualset3
114756	1	402479	13	NULL	NULL	0	NULL	76-year-old man	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A 76-year-old man with chronic obstructive pulmonary disease and a smoking history had a 2-cm solitary pulmonary nodule that was likely to be malignant .
	manualset3
114757	2	402479	13	NULL	NULL	0	NULL	chronic obstructive pulmonary disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A 76-year-old man with chronic obstructive pulmonary disease and a smoking history had a 2-cm solitary pulmonary nodule that was likely to be malignant .
	manualset3
114758	3	402479	13	NULL	NULL	0	NULL	history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 76-year-old man with chronic obstructive pulmonary disease and a smoking history had a 2-cm solitary pulmonary nodule that was likely to be malignant .
	manualset3
114759	4	402479	13	NULL	NULL	0	NULL	2-cm solitary pulmonary nodule	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 76-year-old man with chronic obstructive pulmonary disease and a smoking history had a 2-cm solitary pulmonary nodule that was likely to be malignant .
	manualset3
114760	1	402480	13	NULL	NULL	0	NULL	Lymphocytic hypophysitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocytic hypophysitis presenting early in pregnancy .
	manualset3
114761	2	402480	13	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocytic hypophysitis presenting early in pregnancy .
	manualset3
114762	1	402481	13	NULL	NULL	0	NULL	Lymphoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphoma of the lumbar nerve root : case report .
	manualset3
114763	2	402481	13	NULL	NULL	0	NULL	lumbar nerve root 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphoma of the lumbar nerve root : case report .
	manualset3
114764	3	402481	13	NULL	NULL	0	NULL	case report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphoma of the lumbar nerve root : case report .
	manualset3
114765	1	402482	13	NULL	NULL	0	NULL	Lymphomatous cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphomatous cells exhibited surface expression of CXCR4 , the specific receptor of SDF-1alpha .
	manualset3
114766	2	402482	13	NULL	NULL	0	NULL	surface expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphomatous cells exhibited surface expression of CXCR4 , the specific receptor of SDF-1alpha .
	manualset3
114767	3	402482	13	NULL	NULL	0	NULL	CXCR4 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphomatous cells exhibited surface expression of CXCR4 , the specific receptor of SDF-1alpha .
	manualset3
114768	4	402482	13	NULL	NULL	0	NULL	specific receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphomatous cells exhibited surface expression of CXCR4 , the specific receptor of SDF-1alpha .
	manualset3
114769	5	402482	13	NULL	NULL	0	NULL	SDF-1alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphomatous cells exhibited surface expression of CXCR4 , the specific receptor of SDF-1alpha .
	manualset3
114770	1	402483	13	NULL	NULL	0	NULL	Lymphoplasmacytic sclerosing pancreatitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphoplasmacytic sclerosing pancreatitis presenting as a pancreatic head mass in a child : case report and management recommendations .
	manualset3
114771	2	402483	13	NULL	NULL	0	NULL	pancreatic head mass	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphoplasmacytic sclerosing pancreatitis presenting as a pancreatic head mass in a child : case report and management recommendations .
	manualset3
114772	3	402483	13	NULL	NULL	0	NULL	child	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphoplasmacytic sclerosing pancreatitis presenting as a pancreatic head mass in a child : case report and management recommendations .
	manualset3
114773	4	402483	13	NULL	NULL	0	NULL	case report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphoplasmacytic sclerosing pancreatitis presenting as a pancreatic head mass in a child : case report and management recommendations .
	manualset3
114774	5	402483	13	NULL	NULL	0	NULL	management recommendations	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphoplasmacytic sclerosing pancreatitis presenting as a pancreatic head mass in a child : case report and management recommendations .
	manualset3
114775	1	402484	13	NULL	NULL	0	NULL	Lys - ( Leu8 , des-Arg9 ) - bradykinin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lys - ( Leu8 , des-Arg9 ) - bradykinin blocks lipopolysaccharide-induced SHR aorta hyperpolarization by inhibition of Ca ( + + ) - and ATP-dependent K + channels .
	manualset3
114776	2	402484	13	NULL	NULL	0	NULL	lipopolysaccharide-induced SHR aorta hyperpolarization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lys - ( Leu8 , des-Arg9 ) - bradykinin blocks lipopolysaccharide-induced SHR aorta hyperpolarization by inhibition of Ca ( + + ) - and ATP-dependent K + channels .
	manualset3
114777	3	402484	13	NULL	NULL	0	NULL	inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Lys - ( Leu8 , des-Arg9 ) - bradykinin blocks lipopolysaccharide-induced SHR aorta hyperpolarization by inhibition of Ca ( + + ) - and ATP-dependent K + channels .
	manualset3
114778	4	402484	13	NULL	NULL	0	NULL	blocks	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Lys - ( Leu8 , des-Arg9 ) - bradykinin blocks lipopolysaccharide-induced SHR aorta hyperpolarization by inhibition of Ca ( + + ) - and ATP-dependent K + channels .
	manualset3
114779	5	402484	13	NULL	NULL	NULL	NULL	Ca ( + + ) channels	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Lys - ( Leu8 , des-Arg9 ) - bradykinin blocks lipopolysaccharide-induced SHR aorta hyperpolarization by inhibition of Ca ( + + ) - and ATP-dependent K + channels .
	manualset3
114780	6	402484	13	NULL	NULL	NULL	NULL	ATP-dependent K + channels	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Lys - ( Leu8 , des-Arg9 ) - bradykinin blocks lipopolysaccharide-induced SHR aorta hyperpolarization by inhibition of Ca ( + + ) - and ATP-dependent K + channels .
	manualset3
114781	1	402485	13	NULL	NULL	0	NULL	Lysophosphatidylcholine ( lysoPC )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysophosphatidylcholine ( lysoPC ) , which was abundant in Ox-LDL and was found to be transferred from Ox-LDL to endothelial cells , also caused the inhibition of EDR in response to thrombin or acetylcholine but not to A23187 .
	manualset3
114782	2	402485	13	NULL	NULL	0	NULL	Ox-LDL	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysophosphatidylcholine ( lysoPC ) , which was abundant in Ox-LDL and was found to be transferred from Ox-LDL to endothelial cells , also caused the inhibition of EDR in response to thrombin or acetylcholine but not to A23187 .
	manualset3
114783	3	402485	13	NULL	NULL	0	NULL	Ox-LDL	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysophosphatidylcholine ( lysoPC ) , which was abundant in Ox-LDL and was found to be transferred from Ox-LDL to endothelial cells , also caused the inhibition of EDR in response to thrombin or acetylcholine but not to A23187 .
	manualset3
114784	4	402485	13	NULL	NULL	0	NULL	endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysophosphatidylcholine ( lysoPC ) , which was abundant in Ox-LDL and was found to be transferred from Ox-LDL to endothelial cells , also caused the inhibition of EDR in response to thrombin or acetylcholine but not to A23187 .
	manualset3
114785	5	402485	13	NULL	NULL	0	NULL	inhibition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysophosphatidylcholine ( lysoPC ) , which was abundant in Ox-LDL and was found to be transferred from Ox-LDL to endothelial cells , also caused the inhibition of EDR in response to thrombin or acetylcholine but not to A23187 .
	manualset3
114786	6	402485	13	NULL	NULL	0	NULL	EDR	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysophosphatidylcholine ( lysoPC ) , which was abundant in Ox-LDL and was found to be transferred from Ox-LDL to endothelial cells , also caused the inhibition of EDR in response to thrombin or acetylcholine but not to A23187 .
	manualset3
114787	7	402485	13	NULL	NULL	0	NULL	response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysophosphatidylcholine ( lysoPC ) , which was abundant in Ox-LDL and was found to be transferred from Ox-LDL to endothelial cells , also caused the inhibition of EDR in response to thrombin or acetylcholine but not to A23187 .
	manualset3
114788	8	402485	13	NULL	NULL	0	NULL	thrombin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysophosphatidylcholine ( lysoPC ) , which was abundant in Ox-LDL and was found to be transferred from Ox-LDL to endothelial cells , also caused the inhibition of EDR in response to thrombin or acetylcholine but not to A23187 .
	manualset3
114789	9	402485	13	NULL	NULL	0	NULL	acetylcholine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysophosphatidylcholine ( lysoPC ) , which was abundant in Ox-LDL and was found to be transferred from Ox-LDL to endothelial cells , also caused the inhibition of EDR in response to thrombin or acetylcholine but not to A23187 .
	manualset3
114790	10	402485	13	NULL	NULL	0	NULL	A23187	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysophosphatidylcholine ( lysoPC ) , which was abundant in Ox-LDL and was found to be transferred from Ox-LDL to endothelial cells , also caused the inhibition of EDR in response to thrombin or acetylcholine but not to A23187 .
	manualset3
114791	1	402486	13	NULL	NULL	0	NULL	Lysoplasmenylcholine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysoplasmenylcholine was also more potent than lysophosphatidylcholine in perturbing the dynamics of membrane bilayers comprised of phosphatidylcholine as measured by alterations in the steady-state anisotropy of the diphenylhexatriene probe .
	manualset3
114792	2	402486	13	NULL	NULL	0	NULL	lysophosphatidylcholine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysoplasmenylcholine was also more potent than lysophosphatidylcholine in perturbing the dynamics of membrane bilayers comprised of phosphatidylcholine as measured by alterations in the steady-state anisotropy of the diphenylhexatriene probe .
	manualset3
114793	3	402486	13	NULL	NULL	0	NULL	dynamics 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysoplasmenylcholine was also more potent than lysophosphatidylcholine in perturbing the dynamics of membrane bilayers comprised of phosphatidylcholine as measured by alterations in the steady-state anisotropy of the diphenylhexatriene probe .
	manualset3
114794	4	402486	13	NULL	NULL	0	NULL	membrane bilayers 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysoplasmenylcholine was also more potent than lysophosphatidylcholine in perturbing the dynamics of membrane bilayers comprised of phosphatidylcholine as measured by alterations in the steady-state anisotropy of the diphenylhexatriene probe .
	manualset3
114795	5	402486	13	NULL	NULL	0	NULL	phosphatidylcholine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysoplasmenylcholine was also more potent than lysophosphatidylcholine in perturbing the dynamics of membrane bilayers comprised of phosphatidylcholine as measured by alterations in the steady-state anisotropy of the diphenylhexatriene probe .
	manualset3
114796	6	402486	13	NULL	NULL	0	NULL	alterations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysoplasmenylcholine was also more potent than lysophosphatidylcholine in perturbing the dynamics of membrane bilayers comprised of phosphatidylcholine as measured by alterations in the steady-state anisotropy of the diphenylhexatriene probe .
	manualset3
114797	7	402486	13	NULL	NULL	0	NULL	steady-state anisotropy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysoplasmenylcholine was also more potent than lysophosphatidylcholine in perturbing the dynamics of membrane bilayers comprised of phosphatidylcholine as measured by alterations in the steady-state anisotropy of the diphenylhexatriene probe .
	manualset3
114798	8	402486	13	NULL	NULL	0	NULL	diphenylhexatriene probe 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysoplasmenylcholine was also more potent than lysophosphatidylcholine in perturbing the dynamics of membrane bilayers comprised of phosphatidylcholine as measured by alterations in the steady-state anisotropy of the diphenylhexatriene probe .
	manualset3
114799	1	402487	13	NULL	NULL	0	NULL	Lysosomal arylsulfatases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysosomal arylsulfatases of human leukocytes : increment of phosphorylated B variants in chronic myelogenous leukemia .
	manualset3
114800	2	402487	13	NULL	NULL	0	NULL	human leukocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysosomal arylsulfatases of human leukocytes : increment of phosphorylated B variants in chronic myelogenous leukemia .
	manualset3
114801	3	402487	13	NULL	NULL	0	NULL	increment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysosomal arylsulfatases of human leukocytes : increment of phosphorylated B variants in chronic myelogenous leukemia .
	manualset3
114802	4	402487	13	NULL	NULL	0	NULL	phosphorylated B variants	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysosomal arylsulfatases of human leukocytes : increment of phosphorylated B variants in chronic myelogenous leukemia .
	manualset3
114803	5	402487	13	NULL	NULL	0	NULL	chronic myelogenous leukemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysosomal arylsulfatases of human leukocytes : increment of phosphorylated B variants in chronic myelogenous leukemia .
	manualset3
114804	1	402488	13	NULL	NULL	0	NULL	78-year-old white male	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A 78-year-old white male from Iowa in the United States of America receiving the anti- tumor necrois factor ( TNF ) agent infliximab therapy for rheumatoid arthritis developed a cheek ulcer which failed to respond to empiric antibiotic therapy .
	manualset3
114805	2	402488	13	NULL	NULL	0	NULL	Iowa	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A 78-year-old white male from Iowa in the United States of America receiving the anti- tumor necrois factor ( TNF ) agent infliximab therapy for rheumatoid arthritis developed a cheek ulcer which failed to respond to empiric antibiotic therapy .
	manualset3
114806	3	402488	13	NULL	NULL	0	NULL	United States of America	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A 78-year-old white male from Iowa in the United States of America receiving the anti- tumor necrois factor ( TNF ) agent infliximab therapy for rheumatoid arthritis developed a cheek ulcer which failed to respond to empiric antibiotic therapy .
	manualset3
114807	4	402488	13	NULL	NULL	0	NULL	anti- tumor necrois factor ( TNF ) agent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A 78-year-old white male from Iowa in the United States of America receiving the anti- tumor necrois factor ( TNF ) agent infliximab therapy for rheumatoid arthritis developed a cheek ulcer which failed to respond to empiric antibiotic therapy .
	manualset3
114808	5	402488	13	NULL	NULL	0	NULL	infliximab therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A 78-year-old white male from Iowa in the United States of America receiving the anti- tumor necrois factor ( TNF ) agent infliximab therapy for rheumatoid arthritis developed a cheek ulcer which failed to respond to empiric antibiotic therapy .
	manualset3
114809	6	402488	13	NULL	NULL	0	NULL	rheumatoid arthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A 78-year-old white male from Iowa in the United States of America receiving the anti- tumor necrois factor ( TNF ) agent infliximab therapy for rheumatoid arthritis developed a cheek ulcer which failed to respond to empiric antibiotic therapy .
	manualset3
114810	7	402488	13	NULL	NULL	0	NULL	cheek ulcer	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 78-year-old white male from Iowa in the United States of America receiving the anti- tumor necrois factor ( TNF ) agent infliximab therapy for rheumatoid arthritis developed a cheek ulcer which failed to respond to empiric antibiotic therapy .
	manualset3
114811	8	402488	13	NULL	NULL	0	NULL	 empiric antibiotic therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A 78-year-old white male from Iowa in the United States of America receiving the anti- tumor necrois factor ( TNF ) agent infliximab therapy for rheumatoid arthritis developed a cheek ulcer which failed to respond to empiric antibiotic therapy .
	manualset3
114812	1	402489	13	NULL	NULL	0	NULL	Lysosomal beta-mannosidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysosomal beta-mannosidase was purified 160 , 000-fold in 24 % yield from bovine kidney by a four-step purification procedure , which included concanavalin A-Sepharose , immunoaffinity , TSK-butyl and h.p.l.c. cation-exchange chromatography .
	manualset3
114813	2	402489	13	NULL	NULL	0	NULL	160 , 000-fold	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysosomal beta-mannosidase was purified 160 , 000-fold in 24 % yield from bovine kidney by a four-step purification procedure , which included concanavalin A-Sepharose , immunoaffinity , TSK-butyl and h.p.l.c. cation-exchange chromatography .
	manualset3
114814	3	402489	13	NULL	NULL	0	NULL	24 % yield	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysosomal beta-mannosidase was purified 160 , 000-fold in 24 % yield from bovine kidney by a four-step purification procedure , which included concanavalin A-Sepharose , immunoaffinity , TSK-butyl and h.p.l.c. cation-exchange chromatography .
	manualset3
114815	4	402489	13	NULL	NULL	0	NULL	bovine kidney 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysosomal beta-mannosidase was purified 160 , 000-fold in 24 % yield from bovine kidney by a four-step purification procedure , which included concanavalin A-Sepharose , immunoaffinity , TSK-butyl and h.p.l.c. cation-exchange chromatography .
	manualset3
114816	5	402489	13	NULL	NULL	0	NULL	 four-step purification procedure 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysosomal beta-mannosidase was purified 160 , 000-fold in 24 % yield from bovine kidney by a four-step purification procedure , which included concanavalin A-Sepharose , immunoaffinity , TSK-butyl and h.p.l.c. cation-exchange chromatography .
	manualset3
114817	6	402489	13	NULL	NULL	0	NULL	concanavalin A-Sepharose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysosomal beta-mannosidase was purified 160 , 000-fold in 24 % yield from bovine kidney by a four-step purification procedure , which included concanavalin A-Sepharose , immunoaffinity , TSK-butyl and h.p.l.c. cation-exchange chromatography .
	manualset3
114818	7	402489	13	NULL	NULL	0	NULL	immunoaffinity	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysosomal beta-mannosidase was purified 160 , 000-fold in 24 % yield from bovine kidney by a four-step purification procedure , which included concanavalin A-Sepharose , immunoaffinity , TSK-butyl and h.p.l.c. cation-exchange chromatography .
	manualset3
114819	8	402489	13	NULL	NULL	0	NULL	TSK-butyl 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysosomal beta-mannosidase was purified 160 , 000-fold in 24 % yield from bovine kidney by a four-step purification procedure , which included concanavalin A-Sepharose , immunoaffinity , TSK-butyl and h.p.l.c. cation-exchange chromatography .
	manualset3
114820	9	402489	13	NULL	NULL	0	NULL	h.p.l.c. cation-exchange chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysosomal beta-mannosidase was purified 160 , 000-fold in 24 % yield from bovine kidney by a four-step purification procedure , which included concanavalin A-Sepharose , immunoaffinity , TSK-butyl and h.p.l.c. cation-exchange chromatography .
	manualset3
114821	1	402490	13	NULL	NULL	0	NULL	Lysosomotropic reagents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysosomotropic reagents and a proton ionophore reduced the uptake of 59Fe .
	manualset3
114822	2	402490	13	NULL	NULL	0	NULL	proton ionophore 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysosomotropic reagents and a proton ionophore reduced the uptake of 59Fe .
	manualset3
114823	3	402490	13	NULL	NULL	0	NULL	uptake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysosomotropic reagents and a proton ionophore reduced the uptake of 59Fe .
	manualset3
114824	4	402490	13	NULL	NULL	0	NULL	59Fe	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysosomotropic reagents and a proton ionophore reduced the uptake of 59Fe .
	manualset3
114825	1	402491	13	NULL	NULL	0	NULL	M-antigens	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	M-antigens of seven M-types of group A streptococci were used to compare antigenic response in six breeds of rabbits : New Zealand White , New Zealand Red , Dutch , Googy , California , and Palomino .
	manualset3
114826	2	402491	13	NULL	NULL	0	NULL	seven M-types of group A streptococci 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	M-antigens of seven M-types of group A streptococci were used to compare antigenic response in six breeds of rabbits : New Zealand White , New Zealand Red , Dutch , Googy , California , and Palomino .
	manualset3
114827	3	402491	13	NULL	NULL	0	NULL	antigenic response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	M-antigens of seven M-types of group A streptococci were used to compare antigenic response in six breeds of rabbits : New Zealand White , New Zealand Red , Dutch , Googy , California , and Palomino .
	manualset3
114828	4	402491	13	NULL	NULL	0	NULL	six breeds 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	M-antigens of seven M-types of group A streptococci were used to compare antigenic response in six breeds of rabbits : New Zealand White , New Zealand Red , Dutch , Googy , California , and Palomino .
	manualset3
114829	5	402491	13	NULL	NULL	0	NULL	rabbits	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	M-antigens of seven M-types of group A streptococci were used to compare antigenic response in six breeds of rabbits : New Zealand White , New Zealand Red , Dutch , Googy , California , and Palomino .
	manualset3
114830	6	402491	13	NULL	NULL	0	NULL	New Zealand White	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	M-antigens of seven M-types of group A streptococci were used to compare antigenic response in six breeds of rabbits : New Zealand White , New Zealand Red , Dutch , Googy , California , and Palomino .
	manualset3
114831	7	402491	13	NULL	NULL	0	NULL	New Zealand Red	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	M-antigens of seven M-types of group A streptococci were used to compare antigenic response in six breeds of rabbits : New Zealand White , New Zealand Red , Dutch , Googy , California , and Palomino .
	manualset3
114832	8	402491	13	NULL	NULL	0	NULL	Dutch	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	M-antigens of seven M-types of group A streptococci were used to compare antigenic response in six breeds of rabbits : New Zealand White , New Zealand Red , Dutch , Googy , California , and Palomino .
	manualset3
114833	9	402491	13	NULL	NULL	0	NULL	Googy	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	M-antigens of seven M-types of group A streptococci were used to compare antigenic response in six breeds of rabbits : New Zealand White , New Zealand Red , Dutch , Googy , California , and Palomino .
	manualset3
114834	10	402491	13	NULL	NULL	0	NULL	California	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	M-antigens of seven M-types of group A streptococci were used to compare antigenic response in six breeds of rabbits : New Zealand White , New Zealand Red , Dutch , Googy , California , and Palomino .
	manualset3
114835	11	402491	13	NULL	NULL	0	NULL	Palomino	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	M-antigens of seven M-types of group A streptococci were used to compare antigenic response in six breeds of rabbits : New Zealand White , New Zealand Red , Dutch , Googy , California , and Palomino .
	manualset3
114836	1	402492	13	NULL	NULL	0	NULL	M. vaccae vaccine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	M. vaccae vaccine is a candidate for the prevention of tuberculosis in HIV infection .
	manualset3
114837	2	402492	13	NULL	NULL	0	NULL	candidate	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	M. vaccae vaccine is a candidate for the prevention of tuberculosis in HIV infection .
	manualset3
114838	3	402492	13	NULL	NULL	0	NULL	prevention 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	M. vaccae vaccine is a candidate for the prevention of tuberculosis in HIV infection .
	manualset3
114839	4	402492	13	NULL	NULL	0	NULL	tuberculosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	M. vaccae vaccine is a candidate for the prevention of tuberculosis in HIV infection .
	manualset3
114840	5	402492	13	NULL	NULL	0	NULL	HIV infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	M. vaccae vaccine is a candidate for the prevention of tuberculosis in HIV infection .
	manualset3
114841	1	402493	13	NULL	NULL	0	NULL	M. xanthognathus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	M. xanthognathus hemolysate was considerably less soluble than those of M. oeconomus and M. pennsylvanicus pullatus which had essentially the same solubility .
	manualset3
114842	2	402493	13	NULL	NULL	0	NULL	hemolysate	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	M. xanthognathus hemolysate was considerably less soluble than those of M. oeconomus and M. pennsylvanicus pullatus which had essentially the same solubility .
	manualset3
114843	3	402493	13	NULL	NULL	0	NULL	M. oeconomus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	M. xanthognathus hemolysate was considerably less soluble than those of M. oeconomus and M. pennsylvanicus pullatus which had essentially the same solubility .
	manualset3
114844	4	402493	13	NULL	NULL	0	NULL	M. pennsylvanicus pullatus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	M. xanthognathus hemolysate was considerably less soluble than those of M. oeconomus and M. pennsylvanicus pullatus which had essentially the same solubility .
	manualset3
114845	5	402493	13	NULL	NULL	0	NULL	solubility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	M. xanthognathus hemolysate was considerably less soluble than those of M. oeconomus and M. pennsylvanicus pullatus which had essentially the same solubility .
	manualset3
114846	1	402494	13	NULL	NULL	0	NULL	M1 multivoxel patterns  	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	M1 multivoxel patterns of functional MRI activation are more correlated during repeated hand movements to the same targets than to greatly differing ones , and therefore potentially contain information about movement direction .
	manualset3
114847	2	402494	13	NULL	NULL	0	NULL	MRI activation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	M1 multivoxel patterns of functional MRI activation are more correlated during repeated hand movements to the same targets than to greatly differing ones , and therefore potentially contain information about movement direction .
	manualset3
114848	3	402494	13	NULL	NULL	0	NULL	hand movements	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	M1 multivoxel patterns of functional MRI activation are more correlated during repeated hand movements to the same targets than to greatly differing ones , and therefore potentially contain information about movement direction .
	manualset3
114849	4	402494	13	NULL	NULL	0	NULL	targets	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	M1 multivoxel patterns of functional MRI activation are more correlated during repeated hand movements to the same targets than to greatly differing ones , and therefore potentially contain information about movement direction .
	manualset3
114850	5	402494	13	NULL	NULL	0	NULL	information	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	M1 multivoxel patterns of functional MRI activation are more correlated during repeated hand movements to the same targets than to greatly differing ones , and therefore potentially contain information about movement direction .
	manualset3
114851	6	402494	13	NULL	NULL	0	NULL	movement direction	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	M1 multivoxel patterns of functional MRI activation are more correlated during repeated hand movements to the same targets than to greatly differing ones , and therefore potentially contain information about movement direction .
	manualset3
114852	1	402495	13	NULL	NULL	0	NULL	M112 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	M112 protein , like M15 protein , can be activated by anti-beta-galactosidase but to a much higher level .
	manualset3
114853	2	402495	13	NULL	NULL	0	NULL	like M15 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	M112 protein , like M15 protein , can be activated by anti-beta-galactosidase but to a much higher level .
	manualset3
114854	3	402495	13	NULL	NULL	0	NULL	anti-beta-galactosidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	M112 protein , like M15 protein , can be activated by anti-beta-galactosidase but to a much higher level .
	manualset3
114855	4	402495	13	NULL	NULL	0	NULL	higher level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	M112 protein , like M15 protein , can be activated by anti-beta-galactosidase but to a much higher level .
	manualset3
114856	1	402496	13	NULL	NULL	0	NULL	MA treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	MA treatment inhibited body , but not brain weight gain , resulting in hippocampal weights that were heavier in the MA-treated animals when expressed as a percent of body weight .
	manualset3
114857	2	402496	13	NULL	NULL	0	NULL	body weight gain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MA treatment inhibited body , but not brain weight gain , resulting in hippocampal weights that were heavier in the MA-treated animals when expressed as a percent of body weight .
	manualset3
114858	3	402496	13	NULL	NULL	0	NULL	brain weight gain 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MA treatment inhibited body , but not brain weight gain , resulting in hippocampal weights that were heavier in the MA-treated animals when expressed as a percent of body weight .
	manualset3
114859	4	402496	13	NULL	NULL	0	NULL	hippocampal weights	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MA treatment inhibited body , but not brain weight gain , resulting in hippocampal weights that were heavier in the MA-treated animals when expressed as a percent of body weight .
	manualset3
114860	5	402496	13	NULL	NULL	0	NULL	MA-treated animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	MA treatment inhibited body , but not brain weight gain , resulting in hippocampal weights that were heavier in the MA-treated animals when expressed as a percent of body weight .
	manualset3
114861	6	402496	13	NULL	NULL	0	NULL	 percent of body weight	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MA treatment inhibited body , but not brain weight gain , resulting in hippocampal weights that were heavier in the MA-treated animals when expressed as a percent of body weight .
	manualset3
114862	1	402497	13	NULL	NULL	0	NULL	 B-cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A B-cell , Burkitt-type lymphoma , diffusely affecting the peripheral nerves and intramuscular nerve branches was diagnosed in a 4-year-old domestic shorthair cat with a chronic progressive history of flaccid tetraparesis and generalized muscle atrophy .
	manualset3
114863	2	402497	13	NULL	NULL	0	NULL	Burkitt-type lymphoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A B-cell , Burkitt-type lymphoma , diffusely affecting the peripheral nerves and intramuscular nerve branches was diagnosed in a 4-year-old domestic shorthair cat with a chronic progressive history of flaccid tetraparesis and generalized muscle atrophy .
	manualset3
114864	3	402497	13	NULL	NULL	0	NULL	peripheral nerves	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A B-cell , Burkitt-type lymphoma , diffusely affecting the peripheral nerves and intramuscular nerve branches was diagnosed in a 4-year-old domestic shorthair cat with a chronic progressive history of flaccid tetraparesis and generalized muscle atrophy .
	manualset3
114865	4	402497	13	NULL	NULL	0	NULL	 intramuscular nerve branches	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A B-cell , Burkitt-type lymphoma , diffusely affecting the peripheral nerves and intramuscular nerve branches was diagnosed in a 4-year-old domestic shorthair cat with a chronic progressive history of flaccid tetraparesis and generalized muscle atrophy .
	manualset3
114866	5	402497	13	NULL	NULL	0	NULL	4-year-old 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A B-cell , Burkitt-type lymphoma , diffusely affecting the peripheral nerves and intramuscular nerve branches was diagnosed in a 4-year-old domestic shorthair cat with a chronic progressive history of flaccid tetraparesis and generalized muscle atrophy .
	manualset3
114867	6	402497	13	NULL	NULL	0	NULL	domestic shorthair cat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A B-cell , Burkitt-type lymphoma , diffusely affecting the peripheral nerves and intramuscular nerve branches was diagnosed in a 4-year-old domestic shorthair cat with a chronic progressive history of flaccid tetraparesis and generalized muscle atrophy .
	manualset3
114868	7	402497	13	NULL	NULL	0	NULL	chronic progressive history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A B-cell , Burkitt-type lymphoma , diffusely affecting the peripheral nerves and intramuscular nerve branches was diagnosed in a 4-year-old domestic shorthair cat with a chronic progressive history of flaccid tetraparesis and generalized muscle atrophy .
	manualset3
114869	8	402497	13	NULL	NULL	0	NULL	flaccid tetraparesis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A B-cell , Burkitt-type lymphoma , diffusely affecting the peripheral nerves and intramuscular nerve branches was diagnosed in a 4-year-old domestic shorthair cat with a chronic progressive history of flaccid tetraparesis and generalized muscle atrophy .
	manualset3
114870	9	402497	13	NULL	NULL	0	NULL	generalized muscle atrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A B-cell , Burkitt-type lymphoma , diffusely affecting the peripheral nerves and intramuscular nerve branches was diagnosed in a 4-year-old domestic shorthair cat with a chronic progressive history of flaccid tetraparesis and generalized muscle atrophy .
	manualset3
114871	1	402498	13	NULL	NULL	NULL	NULL	MAAs	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	MAAs are present in the form of oligosaccharide-linked molecules .
	manualset3
114872	2	402498	13	NULL	NULL	0	NULL	form 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MAAs are present in the form of oligosaccharide-linked molecules .
	manualset3
114873	3	402498	13	NULL	NULL	0	NULL	 oligosaccharide-linked molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	MAAs are present in the form of oligosaccharide-linked molecules .
	manualset3
114874	1	402499	13	NULL	NULL	NULL	NULL	MABDOS	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	MABDOS , a program for performing internal radionuclide dosimetry , addresses this shortcoming .
	manualset3
114875	2	402499	13	NULL	NULL	NULL	NULL	program	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	MABDOS , a program for performing internal radionuclide dosimetry , addresses this shortcoming .
	manualset3
114876	3	402499	13	NULL	NULL	NULL	NULL	 radionuclide dosimetry	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	MABDOS , a program for performing internal radionuclide dosimetry , addresses this shortcoming .
	manualset3
114877	1	402500	13	NULL	NULL	0	NULL	MAGE-B5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	MAGE-B5 , MAGE-B6 , MAGE-C2 , and MAGE-C3 : four new members of the MAGE family with tumor-specific expression .
	manualset3
114878	2	402500	13	NULL	NULL	0	NULL	MAGE-B6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	MAGE-B5 , MAGE-B6 , MAGE-C2 , and MAGE-C3 : four new members of the MAGE family with tumor-specific expression .
	manualset3
114879	3	402500	13	NULL	NULL	0	NULL	MAGE-C2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	MAGE-B5 , MAGE-B6 , MAGE-C2 , and MAGE-C3 : four new members of the MAGE family with tumor-specific expression .
	manualset3
114880	4	402500	13	NULL	NULL	0	NULL	 MAGE-C3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	MAGE-B5 , MAGE-B6 , MAGE-C2 , and MAGE-C3 : four new members of the MAGE family with tumor-specific expression .
	manualset3
114881	5	402500	13	NULL	NULL	0	NULL	four new members 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	MAGE-B5 , MAGE-B6 , MAGE-C2 , and MAGE-C3 : four new members of the MAGE family with tumor-specific expression .
	manualset3
114882	6	402500	13	NULL	NULL	0	NULL	MAGE family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	MAGE-B5 , MAGE-B6 , MAGE-C2 , and MAGE-C3 : four new members of the MAGE family with tumor-specific expression .
	manualset3
114883	7	402500	13	NULL	NULL	0	NULL	tumor-specific expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MAGE-B5 , MAGE-B6 , MAGE-C2 , and MAGE-C3 : four new members of the MAGE family with tumor-specific expression .
	manualset3
114933	1	402501	13	NULL	NULL	NULL	NULL	MAIN OUTCOME MEASURES	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	MAIN OUTCOME MEASURES Demographics , laboratory studies , type of intervention , transfusion status , need for hematology consultation , type of coagulopathy , and disposition were recorded .
	manualset3
114934	2	402501	13	NULL	NULL	NULL	NULL	laboratory studies	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	MAIN OUTCOME MEASURES Demographics , laboratory studies , type of intervention , transfusion status , need for hematology consultation , type of coagulopathy , and disposition were recorded .
	manualset3
114935	3	402501	13	NULL	NULL	0	NULL	type of intervention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	MAIN OUTCOME MEASURES Demographics , laboratory studies , type of intervention , transfusion status , need for hematology consultation , type of coagulopathy , and disposition were recorded .
	manualset3
114936	4	402501	13	NULL	NULL	0	NULL	Demographics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MAIN OUTCOME MEASURES Demographics , laboratory studies , type of intervention , transfusion status , need for hematology consultation , type of coagulopathy , and disposition were recorded .
	manualset3
114937	5	402501	13	NULL	NULL	0	NULL	transfusion status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MAIN OUTCOME MEASURES Demographics , laboratory studies , type of intervention , transfusion status , need for hematology consultation , type of coagulopathy , and disposition were recorded .
	manualset3
114938	6	402501	13	NULL	NULL	0	NULL	need	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MAIN OUTCOME MEASURES Demographics , laboratory studies , type of intervention , transfusion status , need for hematology consultation , type of coagulopathy , and disposition were recorded .
	manualset3
114939	7	402501	13	NULL	NULL	0	NULL	hematology consultation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	MAIN OUTCOME MEASURES Demographics , laboratory studies , type of intervention , transfusion status , need for hematology consultation , type of coagulopathy , and disposition were recorded .
	manualset3
114940	8	402501	13	NULL	NULL	0	NULL	type of coagulopathy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MAIN OUTCOME MEASURES Demographics , laboratory studies , type of intervention , transfusion status , need for hematology consultation , type of coagulopathy , and disposition were recorded .
	manualset3
114941	9	402501	13	NULL	NULL	0	NULL	disposition 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MAIN OUTCOME MEASURES Demographics , laboratory studies , type of intervention , transfusion status , need for hematology consultation , type of coagulopathy , and disposition were recorded .
	manualset3
114942	1	402502	13	NULL	NULL	0	NULL	MATERIAL AND METHODS 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	MATERIAL AND METHODS : Four equal groups ( 100 people each ) were studied by an anonymous questionnaire .
	manualset3
114943	2	402502	13	NULL	NULL	0	NULL	Four equal groups ( 100 people each ) 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	MATERIAL AND METHODS : Four equal groups ( 100 people each ) were studied by an anonymous questionnaire .
	manualset3
114944	3	402502	13	NULL	NULL	0	NULL	anonymous questionnaire	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	MATERIAL AND METHODS : Four equal groups ( 100 people each ) were studied by an anonymous questionnaire .
	manualset3
114945	1	402503	13	NULL	NULL	0	NULL	MCC	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	MCC mutants exhibited increased resistance to heat stress compared with wild-type flies .
	manualset3
114946	2	402503	13	NULL	NULL	0	NULL	mutants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	MCC mutants exhibited increased resistance to heat stress compared with wild-type flies .
	manualset3
114947	3	402503	13	NULL	NULL	0	NULL	resistance 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MCC mutants exhibited increased resistance to heat stress compared with wild-type flies .
	manualset3
114948	4	402503	13	NULL	NULL	0	NULL	heat stress	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	MCC mutants exhibited increased resistance to heat stress compared with wild-type flies .
	manualset3
114949	5	402503	13	NULL	NULL	0	NULL	wild-type flies	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	MCC mutants exhibited increased resistance to heat stress compared with wild-type flies .
	manualset3
114950	1	402504	13	NULL	NULL	0	NULL	MDC 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	MDC were harvested from mice hindleg muscle , transfected with a plasmid encoding for beta-galactosidase , and placed into single-layer SIS cell culture inserts .
	manualset3
114951	2	402504	13	NULL	NULL	0	NULL	mice hindleg muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	MDC were harvested from mice hindleg muscle , transfected with a plasmid encoding for beta-galactosidase , and placed into single-layer SIS cell culture inserts .
	manualset3
114952	3	402504	13	NULL	NULL	0	NULL	plasmid	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	MDC were harvested from mice hindleg muscle , transfected with a plasmid encoding for beta-galactosidase , and placed into single-layer SIS cell culture inserts .
	manualset3
114953	4	402504	13	NULL	NULL	0	NULL	encoding 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MDC were harvested from mice hindleg muscle , transfected with a plasmid encoding for beta-galactosidase , and placed into single-layer SIS cell culture inserts .
	manualset3
114954	5	402504	13	NULL	NULL	0	NULL	beta-galactosidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	MDC were harvested from mice hindleg muscle , transfected with a plasmid encoding for beta-galactosidase , and placed into single-layer SIS cell culture inserts .
	manualset3
114955	6	402504	13	NULL	NULL	0	NULL	single-layer SIS cell culture inserts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	MDC were harvested from mice hindleg muscle , transfected with a plasmid encoding for beta-galactosidase , and placed into single-layer SIS cell culture inserts .
	manualset3
114956	1	402505	13	NULL	NULL	0	NULL	MDF 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	MDF produced a rapid reduction in the serum iron levels with accumulation of iron in spleen .
	manualset3
114957	2	402505	13	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MDF produced a rapid reduction in the serum iron levels with accumulation of iron in spleen .
	manualset3
114958	3	402505	13	NULL	NULL	0	NULL	serum iron levels 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MDF produced a rapid reduction in the serum iron levels with accumulation of iron in spleen .
	manualset3
114959	4	402505	13	NULL	NULL	0	NULL	accumulation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MDF produced a rapid reduction in the serum iron levels with accumulation of iron in spleen .
	manualset3
114960	5	402505	13	NULL	NULL	0	NULL	iron	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	MDF produced a rapid reduction in the serum iron levels with accumulation of iron in spleen .
	manualset3
114961	6	402505	13	NULL	NULL	0	NULL	spleen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	MDF produced a rapid reduction in the serum iron levels with accumulation of iron in spleen .
	manualset3
114962	1	402506	13	NULL	NULL	0	NULL	MEASUREMENT 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	MEASUREMENT OF ABDOMINAL FAT DEPOTS : Various anthropometric indicators have been suggested for measuring body fat distribution .
	manualset3
114963	2	402506	13	NULL	NULL	0	NULL	ABDOMINAL FAT DEPOTS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MEASUREMENT OF ABDOMINAL FAT DEPOTS : Various anthropometric indicators have been suggested for measuring body fat distribution .
	manualset3
114964	3	402506	13	NULL	NULL	0	NULL	anthropometric indicators 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MEASUREMENT OF ABDOMINAL FAT DEPOTS : Various anthropometric indicators have been suggested for measuring body fat distribution .
	manualset3
114965	4	402506	13	NULL	NULL	0	NULL	body fat distribution	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MEASUREMENT OF ABDOMINAL FAT DEPOTS : Various anthropometric indicators have been suggested for measuring body fat distribution .
	manualset3
114966	1	402507	13	NULL	NULL	0	NULL	MEEKC methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	MEEKC methods , based on 2-hexanol and cyclohexanol as cosurfactant were validated and successfully applied to the analysis of catechins and caffeine in commercial green tea products .
	manualset3
114967	2	402507	13	NULL	NULL	0	NULL	2-hexanol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	MEEKC methods , based on 2-hexanol and cyclohexanol as cosurfactant were validated and successfully applied to the analysis of catechins and caffeine in commercial green tea products .
	manualset3
114968	3	402507	13	NULL	NULL	0	NULL	cyclohexanol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	MEEKC methods , based on 2-hexanol and cyclohexanol as cosurfactant were validated and successfully applied to the analysis of catechins and caffeine in commercial green tea products .
	manualset3
114969	4	402507	13	NULL	NULL	0	NULL	cosurfactant	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	MEEKC methods , based on 2-hexanol and cyclohexanol as cosurfactant were validated and successfully applied to the analysis of catechins and caffeine in commercial green tea products .
	manualset3
114970	5	402507	13	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	MEEKC methods , based on 2-hexanol and cyclohexanol as cosurfactant were validated and successfully applied to the analysis of catechins and caffeine in commercial green tea products .
	manualset3
114971	6	402507	13	NULL	NULL	0	NULL	catechins 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	MEEKC methods , based on 2-hexanol and cyclohexanol as cosurfactant were validated and successfully applied to the analysis of catechins and caffeine in commercial green tea products .
	manualset3
114972	7	402507	13	NULL	NULL	0	NULL	caffeine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	MEEKC methods , based on 2-hexanol and cyclohexanol as cosurfactant were validated and successfully applied to the analysis of catechins and caffeine in commercial green tea products .
	manualset3
114973	8	402507	13	NULL	NULL	0	NULL	green tea products	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	MEEKC methods , based on 2-hexanol and cyclohexanol as cosurfactant were validated and successfully applied to the analysis of catechins and caffeine in commercial green tea products .
	manualset3
114974	1	402508	13	NULL	NULL	0	NULL	METHODS	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	METHODS : The impact of PCOS , as well as the impact of IR and BMI on the hormonal , metabolic and hemostatic key variables will be analyzed combining conventional , molecular techniques and selected gene analysis .
	manualset3
114975	2	402508	13	NULL	NULL	0	NULL	impact of PCOS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	METHODS : The impact of PCOS , as well as the impact of IR and BMI on the hormonal , metabolic and hemostatic key variables will be analyzed combining conventional , molecular techniques and selected gene analysis .
	manualset3
114976	3	402508	13	NULL	NULL	0	NULL	impact of IR	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	METHODS : The impact of PCOS , as well as the impact of IR and BMI on the hormonal , metabolic and hemostatic key variables will be analyzed combining conventional , molecular techniques and selected gene analysis .
	manualset3
114977	4	402508	13	NULL	NULL	0	NULL	BMI	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	METHODS : The impact of PCOS , as well as the impact of IR and BMI on the hormonal , metabolic and hemostatic key variables will be analyzed combining conventional , molecular techniques and selected gene analysis .
	manualset3
114978	5	402508	13	NULL	NULL	0	NULL	hormonal variables	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	METHODS : The impact of PCOS , as well as the impact of IR and BMI on the hormonal , metabolic and hemostatic key variables will be analyzed combining conventional , molecular techniques and selected gene analysis .
	manualset3
114979	6	402508	13	NULL	NULL	0	NULL	metabolic variables	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	METHODS : The impact of PCOS , as well as the impact of IR and BMI on the hormonal , metabolic and hemostatic key variables will be analyzed combining conventional , molecular techniques and selected gene analysis .
	manualset3
114980	7	402508	13	NULL	NULL	0	NULL	hemostatic key variables	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	METHODS : The impact of PCOS , as well as the impact of IR and BMI on the hormonal , metabolic and hemostatic key variables will be analyzed combining conventional , molecular techniques and selected gene analysis .
	manualset3
114981	8	402508	13	NULL	NULL	0	NULL	molecular techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	METHODS : The impact of PCOS , as well as the impact of IR and BMI on the hormonal , metabolic and hemostatic key variables will be analyzed combining conventional , molecular techniques and selected gene analysis .
	manualset3
114982	9	402508	13	NULL	NULL	0	NULL	gene analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	METHODS : The impact of PCOS , as well as the impact of IR and BMI on the hormonal , metabolic and hemostatic key variables will be analyzed combining conventional , molecular techniques and selected gene analysis .
	manualset3
114983	1	402509	13	NULL	NULL	0	NULL	BIPAP system	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A BIPAP system can be set up either as a continuous flow system , or as a demand valve system .
	manualset3
114984	2	402509	13	NULL	NULL	0	NULL	continuous flow system	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A BIPAP system can be set up either as a continuous flow system , or as a demand valve system .
	manualset3
114985	3	402509	13	NULL	NULL	0	NULL	demand valve system	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A BIPAP system can be set up either as a continuous flow system , or as a demand valve system .
	manualset3
114986	1	402510	13	NULL	NULL	0	NULL	METHODS	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	METHODS AND SUBJECTS : The atrial fibrillation and flutter outcomes and risk determination investigation is a prospective , observational cohort study to develop a multivariable clinical prediction rule that accurately estimates risk for adverse outcomes in patients presenting to the ED with symptomatic AF .
	manualset3
114987	2	402510	13	NULL	NULL	0	NULL	SUBJECTS	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	METHODS AND SUBJECTS : The atrial fibrillation and flutter outcomes and risk determination investigation is a prospective , observational cohort study to develop a multivariable clinical prediction rule that accurately estimates risk for adverse outcomes in patients presenting to the ED with symptomatic AF .
	manualset3
114988	3	402510	13	NULL	NULL	0	NULL	atrial fibrillation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	METHODS AND SUBJECTS : The atrial fibrillation and flutter outcomes and risk determination investigation is a prospective , observational cohort study to develop a multivariable clinical prediction rule that accurately estimates risk for adverse outcomes in patients presenting to the ED with symptomatic AF .
	manualset3
114989	4	402510	13	NULL	NULL	0	NULL	flutter outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	METHODS AND SUBJECTS : The atrial fibrillation and flutter outcomes and risk determination investigation is a prospective , observational cohort study to develop a multivariable clinical prediction rule that accurately estimates risk for adverse outcomes in patients presenting to the ED with symptomatic AF .
	manualset3
114990	5	402510	13	NULL	NULL	0	NULL	risk determination 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	METHODS AND SUBJECTS : The atrial fibrillation and flutter outcomes and risk determination investigation is a prospective , observational cohort study to develop a multivariable clinical prediction rule that accurately estimates risk for adverse outcomes in patients presenting to the ED with symptomatic AF .
	manualset3
114991	6	402510	13	NULL	NULL	0	NULL	investigation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	METHODS AND SUBJECTS : The atrial fibrillation and flutter outcomes and risk determination investigation is a prospective , observational cohort study to develop a multivariable clinical prediction rule that accurately estimates risk for adverse outcomes in patients presenting to the ED with symptomatic AF .
	manualset3
114992	7	402510	13	NULL	NULL	0	NULL	cohort study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	METHODS AND SUBJECTS : The atrial fibrillation and flutter outcomes and risk determination investigation is a prospective , observational cohort study to develop a multivariable clinical prediction rule that accurately estimates risk for adverse outcomes in patients presenting to the ED with symptomatic AF .
	manualset3
114993	8	402510	13	NULL	NULL	0	NULL	multivariable clinical prediction rule	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	METHODS AND SUBJECTS : The atrial fibrillation and flutter outcomes and risk determination investigation is a prospective , observational cohort study to develop a multivariable clinical prediction rule that accurately estimates risk for adverse outcomes in patients presenting to the ED with symptomatic AF .
	manualset3
114994	9	402510	13	NULL	NULL	0	NULL	risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	METHODS AND SUBJECTS : The atrial fibrillation and flutter outcomes and risk determination investigation is a prospective , observational cohort study to develop a multivariable clinical prediction rule that accurately estimates risk for adverse outcomes in patients presenting to the ED with symptomatic AF .
	manualset3
114995	10	402510	13	NULL	NULL	0	NULL	adverse outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	METHODS AND SUBJECTS : The atrial fibrillation and flutter outcomes and risk determination investigation is a prospective , observational cohort study to develop a multivariable clinical prediction rule that accurately estimates risk for adverse outcomes in patients presenting to the ED with symptomatic AF .
	manualset3
114996	11	402510	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	METHODS AND SUBJECTS : The atrial fibrillation and flutter outcomes and risk determination investigation is a prospective , observational cohort study to develop a multivariable clinical prediction rule that accurately estimates risk for adverse outcomes in patients presenting to the ED with symptomatic AF .
	manualset3
114997	12	402510	13	NULL	NULL	0	NULL	ED	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	METHODS AND SUBJECTS : The atrial fibrillation and flutter outcomes and risk determination investigation is a prospective , observational cohort study to develop a multivariable clinical prediction rule that accurately estimates risk for adverse outcomes in patients presenting to the ED with symptomatic AF .
	manualset3
114998	13	402510	13	NULL	NULL	0	NULL	symptomatic AF	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	METHODS AND SUBJECTS : The atrial fibrillation and flutter outcomes and risk determination investigation is a prospective , observational cohort study to develop a multivariable clinical prediction rule that accurately estimates risk for adverse outcomes in patients presenting to the ED with symptomatic AF .
	manualset3
114999	1	402511	13	NULL	NULL	0	NULL	MG-dependent O ( 2 ) uptake 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MG-dependent O ( 2 ) uptake was inhibited by 3 - ( 3 , 4-dichlorophenyl ) -1 , 1 - dimethylurea ( DCMU ) and 2 , 5-dibromo-3-methyl-6-isopropyl-p-benzoquinone ( DBMIB ) .
	manualset3
115000	2	402511	13	NULL	NULL	0	NULL	3 - ( 3 , 4-dichlorophenyl ) -1 , 1 - dimethylurea ( DCMU )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	MG-dependent O ( 2 ) uptake was inhibited by 3 - ( 3 , 4-dichlorophenyl ) -1 , 1 - dimethylurea ( DCMU ) and 2 , 5-dibromo-3-methyl-6-isopropyl-p-benzoquinone ( DBMIB ) .
	manualset3
115001	3	402511	13	NULL	NULL	0	NULL	2 , 5-dibromo-3-methyl-6-isopropyl-p-benzoquinone ( DBMIB ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	MG-dependent O ( 2 ) uptake was inhibited by 3 - ( 3 , 4-dichlorophenyl ) -1 , 1 - dimethylurea ( DCMU ) and 2 , 5-dibromo-3-methyl-6-isopropyl-p-benzoquinone ( DBMIB ) .
	manualset3
115002	1	402512	13	NULL	NULL	0	NULL	MG132	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	MG132 also induced apoptosis , which was accompanied by the loss of mitochondrial membrane potential ( MMP ; Deltapsi ( m ) ) .
	manualset3
115003	2	402512	13	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MG132 also induced apoptosis , which was accompanied by the loss of mitochondrial membrane potential ( MMP ; Deltapsi ( m ) ) .
	manualset3
115004	3	402512	13	NULL	NULL	0	NULL	loss 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MG132 also induced apoptosis , which was accompanied by the loss of mitochondrial membrane potential ( MMP ; Deltapsi ( m ) ) .
	manualset3
115005	4	402512	13	NULL	NULL	0	NULL	mitochondrial membrane potential	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	MG132 also induced apoptosis , which was accompanied by the loss of mitochondrial membrane potential ( MMP ; Deltapsi ( m ) ) .
	manualset3
115006	5	402512	13	NULL	NULL	0	NULL	MMP ; Deltapsi ( m )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	MG132 also induced apoptosis , which was accompanied by the loss of mitochondrial membrane potential ( MMP ; Deltapsi ( m ) ) .
	manualset3
115007	1	402513	13	NULL	NULL	0	NULL	MGS	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	MGS exchange information with community members through a number of interspecies signalling systems including AI-2 and contact dependent mechanisms .
	manualset3
115008	2	402513	13	NULL	NULL	0	NULL	exchange	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MGS exchange information with community members through a number of interspecies signalling systems including AI-2 and contact dependent mechanisms .
	manualset3
115009	3	402513	13	NULL	NULL	0	NULL	information	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MGS exchange information with community members through a number of interspecies signalling systems including AI-2 and contact dependent mechanisms .
	manualset3
115010	4	402513	13	NULL	NULL	0	NULL	community members	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	MGS exchange information with community members through a number of interspecies signalling systems including AI-2 and contact dependent mechanisms .
	manualset3
115011	5	402513	13	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	MGS exchange information with community members through a number of interspecies signalling systems including AI-2 and contact dependent mechanisms .
	manualset3
115012	6	402513	13	NULL	NULL	0	NULL	interspecies signalling systems	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MGS exchange information with community members through a number of interspecies signalling systems including AI-2 and contact dependent mechanisms .
	manualset3
115013	7	402513	13	NULL	NULL	0	NULL	AI-2	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	MGS exchange information with community members through a number of interspecies signalling systems including AI-2 and contact dependent mechanisms .
	manualset3
115014	8	402513	13	NULL	NULL	0	NULL	 contact dependent mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MGS exchange information with community members through a number of interspecies signalling systems including AI-2 and contact dependent mechanisms .
	manualset3
115015	1	402514	13	NULL	NULL	0	NULL	MHC-I levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	MHC-I levels were reduced in VZV-infected cells , and analyses of intracellular MHC-I revealed accumulation of folded MHC-I in the Golgi region , irrespective of ORF66 expression .
	manualset3
115016	2	402514	13	NULL	NULL	0	NULL	VZV-infected cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	MHC-I levels were reduced in VZV-infected cells , and analyses of intracellular MHC-I revealed accumulation of folded MHC-I in the Golgi region , irrespective of ORF66 expression .
	manualset3
115017	3	402514	13	NULL	NULL	0	NULL	analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	MHC-I levels were reduced in VZV-infected cells , and analyses of intracellular MHC-I revealed accumulation of folded MHC-I in the Golgi region , irrespective of ORF66 expression .
	manualset3
115018	4	402514	13	NULL	NULL	0	NULL	intracellular MHC-I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	MHC-I levels were reduced in VZV-infected cells , and analyses of intracellular MHC-I revealed accumulation of folded MHC-I in the Golgi region , irrespective of ORF66 expression .
	manualset3
115019	5	402514	13	NULL	NULL	0	NULL	accumulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MHC-I levels were reduced in VZV-infected cells , and analyses of intracellular MHC-I revealed accumulation of folded MHC-I in the Golgi region , irrespective of ORF66 expression .
	manualset3
115020	6	402514	13	NULL	NULL	0	NULL	MHC-I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	MHC-I levels were reduced in VZV-infected cells , and analyses of intracellular MHC-I revealed accumulation of folded MHC-I in the Golgi region , irrespective of ORF66 expression .
	manualset3
115021	7	402514	13	NULL	NULL	0	NULL	Golgi region	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	MHC-I levels were reduced in VZV-infected cells , and analyses of intracellular MHC-I revealed accumulation of folded MHC-I in the Golgi region , irrespective of ORF66 expression .
	manualset3
115022	8	402514	13	NULL	NULL	0	NULL	ORF66 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MHC-I levels were reduced in VZV-infected cells , and analyses of intracellular MHC-I revealed accumulation of folded MHC-I in the Golgi region , irrespective of ORF66 expression .
	manualset3
115027	1	402515	13	NULL	NULL	0	NULL	MI 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	MI had the highest sensitivity of 65 % , while LAMP , PCR , MHCT and TBS had sensitivities of 45 , 33 , 38 and 24 % , respectively .
	manualset3
115028	2	402515	13	NULL	NULL	0	NULL	sensitivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MI had the highest sensitivity of 65 % , while LAMP , PCR , MHCT and TBS had sensitivities of 45 , 33 , 38 and 24 % , respectively .
	manualset3
115029	3	402515	13	NULL	NULL	0	NULL	65 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	MI had the highest sensitivity of 65 % , while LAMP , PCR , MHCT and TBS had sensitivities of 45 , 33 , 38 and 24 % , respectively .
	manualset3
115030	4	402515	13	NULL	NULL	0	NULL	LAMP	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	MI had the highest sensitivity of 65 % , while LAMP , PCR , MHCT and TBS had sensitivities of 45 , 33 , 38 and 24 % , respectively .
	manualset3
115031	5	402515	13	NULL	NULL	0	NULL	PCR 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	MI had the highest sensitivity of 65 % , while LAMP , PCR , MHCT and TBS had sensitivities of 45 , 33 , 38 and 24 % , respectively .
	manualset3
115032	6	402515	13	NULL	NULL	0	NULL	MHCT	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	MI had the highest sensitivity of 65 % , while LAMP , PCR , MHCT and TBS had sensitivities of 45 , 33 , 38 and 24 % , respectively .
	manualset3
115033	7	402515	13	NULL	NULL	0	NULL	TBS 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	MI had the highest sensitivity of 65 % , while LAMP , PCR , MHCT and TBS had sensitivities of 45 , 33 , 38 and 24 % , respectively .
	manualset3
115034	8	402515	13	NULL	NULL	0	NULL	sensitivities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MI had the highest sensitivity of 65 % , while LAMP , PCR , MHCT and TBS had sensitivities of 45 , 33 , 38 and 24 % , respectively .
	manualset3
115035	9	402515	13	NULL	NULL	0	NULL	45 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	MI had the highest sensitivity of 65 % , while LAMP , PCR , MHCT and TBS had sensitivities of 45 , 33 , 38 and 24 % , respectively .
	manualset3
115036	10	402515	13	NULL	NULL	0	NULL	33 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	MI had the highest sensitivity of 65 % , while LAMP , PCR , MHCT and TBS had sensitivities of 45 , 33 , 38 and 24 % , respectively .
	manualset3
115037	11	402515	13	NULL	NULL	0	NULL	 38 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	MI had the highest sensitivity of 65 % , while LAMP , PCR , MHCT and TBS had sensitivities of 45 , 33 , 38 and 24 % , respectively .
	manualset3
115038	12	402515	13	NULL	NULL	0	NULL	24 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	MI had the highest sensitivity of 65 % , while LAMP , PCR , MHCT and TBS had sensitivities of 45 , 33 , 38 and 24 % , respectively .
	manualset3
115039	1	402516	13	NULL	NULL	0	NULL	MIF 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	MIF was localized within the epidermis and the vascular area of skin , but diffusely expressed in the entire thickness of colon .
	manualset3
115040	2	402516	13	NULL	NULL	0	NULL	epidermis 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	MIF was localized within the epidermis and the vascular area of skin , but diffusely expressed in the entire thickness of colon .
	manualset3
115041	3	402516	13	NULL	NULL	0	NULL	vascular area of skin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	MIF was localized within the epidermis and the vascular area of skin , but diffusely expressed in the entire thickness of colon .
	manualset3
115042	4	402516	13	NULL	NULL	NULL	NULL	thickness 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	MIF was localized within the epidermis and the vascular area of skin , but diffusely expressed in the entire thickness of colon .
	manualset3
115043	5	402516	13	NULL	NULL	0	NULL	colon	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	MIF was localized within the epidermis and the vascular area of skin , but diffusely expressed in the entire thickness of colon .
	manualset3
115049	1	402517	13	NULL	NULL	0	NULL	MK-7 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	MK-7 was accumulated under microaerobic condition and UQ-10 was accumulated under aerobic condition in M. huakuii 7653R .
	manualset3
115050	2	402517	13	NULL	NULL	0	NULL	microaerobic condition	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	MK-7 was accumulated under microaerobic condition and UQ-10 was accumulated under aerobic condition in M. huakuii 7653R .
	manualset3
115051	3	402517	13	NULL	NULL	0	NULL	UQ-10 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	MK-7 was accumulated under microaerobic condition and UQ-10 was accumulated under aerobic condition in M. huakuii 7653R .
	manualset3
115052	4	402517	13	NULL	NULL	0	NULL	aerobic condition	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	MK-7 was accumulated under microaerobic condition and UQ-10 was accumulated under aerobic condition in M. huakuii 7653R .
	manualset3
115053	5	402517	13	NULL	NULL	0	NULL	M. huakuii 7653R 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	MK-7 was accumulated under microaerobic condition and UQ-10 was accumulated under aerobic condition in M. huakuii 7653R .
	manualset3
115054	1	402518	13	NULL	NULL	0	NULL	MK	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	MK and other Theileria species .
	manualset3
115055	2	402518	13	NULL	NULL	0	NULL	Theileria species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	MK and other Theileria species .
	manualset3
115131	1	402519	13	NULL	NULL	0	NULL	MKlp1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	MKlp1 is negatively regulated by Cdk1 phosphorylation during metaphase and becomes activated in anaphase when cleavage-furrow assembly commences .
	manualset3
115132	2	402519	13	NULL	NULL	0	NULL	Cdk1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	MKlp1 is negatively regulated by Cdk1 phosphorylation during metaphase and becomes activated in anaphase when cleavage-furrow assembly commences .
	manualset3
115133	3	402519	13	NULL	NULL	0	NULL	phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MKlp1 is negatively regulated by Cdk1 phosphorylation during metaphase and becomes activated in anaphase when cleavage-furrow assembly commences .
	manualset3
115134	4	402519	13	NULL	NULL	0	NULL	metaphase	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	MKlp1 is negatively regulated by Cdk1 phosphorylation during metaphase and becomes activated in anaphase when cleavage-furrow assembly commences .
	manualset3
115135	5	402519	13	NULL	NULL	0	NULL	anaphase	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	MKlp1 is negatively regulated by Cdk1 phosphorylation during metaphase and becomes activated in anaphase when cleavage-furrow assembly commences .
	manualset3
115136	6	402519	13	NULL	NULL	0	NULL	cleavage-furrow assembly	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MKlp1 is negatively regulated by Cdk1 phosphorylation during metaphase and becomes activated in anaphase when cleavage-furrow assembly commences .
	manualset3
115137	1	402520	13	NULL	NULL	0	NULL	MLO-A5	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	MLO-A5 , late osteoblast cells , were exposed to polymerized silorane ( SilMix ) resin ( and a standard polymerized bisGMA/TEGDMA methacrylate ( BT ) resin and compared to culture wells without resins as control .
	manualset3
115138	2	402520	13	NULL	NULL	0	NULL	late osteoblast cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	MLO-A5 , late osteoblast cells , were exposed to polymerized silorane ( SilMix ) resin ( and a standard polymerized bisGMA/TEGDMA methacrylate ( BT ) resin and compared to culture wells without resins as control .
	manualset3
115139	3	402520	13	NULL	NULL	0	NULL	silorane ( SilMix ) resin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	MLO-A5 , late osteoblast cells , were exposed to polymerized silorane ( SilMix ) resin ( and a standard polymerized bisGMA/TEGDMA methacrylate ( BT ) resin and compared to culture wells without resins as control .
	manualset3
115140	4	402520	13	NULL	NULL	0	NULL	bisGMA/TEGDMA methacrylate ( BT ) resin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	MLO-A5 , late osteoblast cells , were exposed to polymerized silorane ( SilMix ) resin ( and a standard polymerized bisGMA/TEGDMA methacrylate ( BT ) resin and compared to culture wells without resins as control .
	manualset3
115141	5	402520	13	NULL	NULL	0	NULL	culture wells	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	MLO-A5 , late osteoblast cells , were exposed to polymerized silorane ( SilMix ) resin ( and a standard polymerized bisGMA/TEGDMA methacrylate ( BT ) resin and compared to culture wells without resins as control .
	manualset3
115142	6	402520	13	NULL	NULL	0	NULL	resins	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	MLO-A5 , late osteoblast cells , were exposed to polymerized silorane ( SilMix ) resin ( and a standard polymerized bisGMA/TEGDMA methacrylate ( BT ) resin and compared to culture wells without resins as control .
	manualset3
115143	1	402521	13	NULL	NULL	0	NULL	MLPA analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	MLPA analysis for the detection of deletions , duplications and complex rearrangements in the dystrophin gene : potential and pitfalls .
	manualset3
115144	2	402521	13	NULL	NULL	0	NULL	detection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MLPA analysis for the detection of deletions , duplications and complex rearrangements in the dystrophin gene : potential and pitfalls .
	manualset3
115145	3	402521	13	NULL	NULL	0	NULL	deletions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MLPA analysis for the detection of deletions , duplications and complex rearrangements in the dystrophin gene : potential and pitfalls .
	manualset3
115146	4	402521	13	NULL	NULL	0	NULL	duplications 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MLPA analysis for the detection of deletions , duplications and complex rearrangements in the dystrophin gene : potential and pitfalls .
	manualset3
115147	5	402521	13	NULL	NULL	0	NULL	complex rearrangements	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MLPA analysis for the detection of deletions , duplications and complex rearrangements in the dystrophin gene : potential and pitfalls .
	manualset3
115148	6	402521	13	NULL	NULL	0	NULL	dystrophin gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	MLPA analysis for the detection of deletions , duplications and complex rearrangements in the dystrophin gene : potential and pitfalls .
	manualset3
115149	7	402521	13	NULL	NULL	0	NULL	pitfalls	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MLPA analysis for the detection of deletions , duplications and complex rearrangements in the dystrophin gene : potential and pitfalls .
	manualset3
115150	1	402522	13	NULL	NULL	0	NULL	MMC 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	MMC interaction with XDH was also assessed by monitoring the ability of MMC to inhibit XDH-mediated uric acid and NADH formation .
	manualset3
115151	2	402522	13	NULL	NULL	0	NULL	interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MMC interaction with XDH was also assessed by monitoring the ability of MMC to inhibit XDH-mediated uric acid and NADH formation .
	manualset3
115152	3	402522	13	NULL	NULL	0	NULL	XDH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	MMC interaction with XDH was also assessed by monitoring the ability of MMC to inhibit XDH-mediated uric acid and NADH formation .
	manualset3
115153	4	402522	13	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MMC interaction with XDH was also assessed by monitoring the ability of MMC to inhibit XDH-mediated uric acid and NADH formation .
	manualset3
115154	5	402522	13	NULL	NULL	0	NULL	MMC	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	MMC interaction with XDH was also assessed by monitoring the ability of MMC to inhibit XDH-mediated uric acid and NADH formation .
	manualset3
115155	6	402522	13	NULL	NULL	0	NULL	XDH-mediated uric acid formation  	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MMC interaction with XDH was also assessed by monitoring the ability of MMC to inhibit XDH-mediated uric acid and NADH formation .
	manualset3
115156	7	402522	13	NULL	NULL	0	NULL	XDH-mediated NADH formation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MMC interaction with XDH was also assessed by monitoring the ability of MMC to inhibit XDH-mediated uric acid and NADH formation .
	manualset3
115157	1	402523	13	NULL	NULL	0	NULL	MMN	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MMN was elicited by the vowel change .
	manualset3
115158	2	402523	13	NULL	NULL	0	NULL	vowel change 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MMN was elicited by the vowel change .
	manualset3
115159	1	402524	13	NULL	NULL	0	NULL	MMP-9	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	MMP-9 and TIMP-1 expressions of all cases were compared statistically with the existing pathological findings and the control group .
	manualset3
115160	2	402524	13	NULL	NULL	0	NULL	TIMP-1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	MMP-9 and TIMP-1 expressions of all cases were compared statistically with the existing pathological findings and the control group .
	manualset3
115161	3	402524	13	NULL	NULL	0	NULL	expressions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MMP-9 and TIMP-1 expressions of all cases were compared statistically with the existing pathological findings and the control group .
	manualset3
115162	4	402524	13	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	MMP-9 and TIMP-1 expressions of all cases were compared statistically with the existing pathological findings and the control group .
	manualset3
115163	5	402524	13	NULL	NULL	0	NULL	pathological findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MMP-9 and TIMP-1 expressions of all cases were compared statistically with the existing pathological findings and the control group .
	manualset3
115164	6	402524	13	NULL	NULL	0	NULL	control group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	MMP-9 and TIMP-1 expressions of all cases were compared statistically with the existing pathological findings and the control group .
	manualset3
115165	1	402525	13	NULL	NULL	0	NULL	MMPs 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	MMPs not only degrade structural proteins , but are also important mediators of cell signaling near or at the cell membrane through exposure of cryptic sites , release of growth factors , and cleavage of receptors .
	manualset3
115166	2	402525	13	NULL	NULL	0	NULL	structural proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	MMPs not only degrade structural proteins , but are also important mediators of cell signaling near or at the cell membrane through exposure of cryptic sites , release of growth factors , and cleavage of receptors .
	manualset3
115167	3	402525	13	NULL	NULL	0	NULL	mediators 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	MMPs not only degrade structural proteins , but are also important mediators of cell signaling near or at the cell membrane through exposure of cryptic sites , release of growth factors , and cleavage of receptors .
	manualset3
115168	4	402525	13	NULL	NULL	0	NULL	cell signaling 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MMPs not only degrade structural proteins , but are also important mediators of cell signaling near or at the cell membrane through exposure of cryptic sites , release of growth factors , and cleavage of receptors .
	manualset3
115169	5	402525	13	NULL	NULL	0	NULL	cell membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	MMPs not only degrade structural proteins , but are also important mediators of cell signaling near or at the cell membrane through exposure of cryptic sites , release of growth factors , and cleavage of receptors .
	manualset3
115170	6	402525	13	NULL	NULL	NULL	NULL	exposure 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	MMPs not only degrade structural proteins , but are also important mediators of cell signaling near or at the cell membrane through exposure of cryptic sites , release of growth factors , and cleavage of receptors .
	manualset3
115171	7	402525	13	NULL	NULL	0	NULL	cryptic sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	MMPs not only degrade structural proteins , but are also important mediators of cell signaling near or at the cell membrane through exposure of cryptic sites , release of growth factors , and cleavage of receptors .
	manualset3
115172	8	402525	13	NULL	NULL	0	NULL	 release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MMPs not only degrade structural proteins , but are also important mediators of cell signaling near or at the cell membrane through exposure of cryptic sites , release of growth factors , and cleavage of receptors .
	manualset3
115173	9	402525	13	NULL	NULL	0	NULL	growth factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	MMPs not only degrade structural proteins , but are also important mediators of cell signaling near or at the cell membrane through exposure of cryptic sites , release of growth factors , and cleavage of receptors .
	manualset3
115174	10	402525	13	NULL	NULL	0	NULL	cleavage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MMPs not only degrade structural proteins , but are also important mediators of cell signaling near or at the cell membrane through exposure of cryptic sites , release of growth factors , and cleavage of receptors .
	manualset3
115175	11	402525	13	NULL	NULL	0	NULL	receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	MMPs not only degrade structural proteins , but are also important mediators of cell signaling near or at the cell membrane through exposure of cryptic sites , release of growth factors , and cleavage of receptors .
	manualset3
115176	1	402526	13	NULL	NULL	0	NULL	MMPs 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	MMPs play an essential role in several normal physiological processes including growth , wound healing and tissue repair .
	manualset3
115177	2	402526	13	NULL	NULL	0	NULL	play	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MMPs play an essential role in several normal physiological processes including growth , wound healing and tissue repair .
	manualset3
115178	3	402526	13	NULL	NULL	0	NULL	essential role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MMPs play an essential role in several normal physiological processes including growth , wound healing and tissue repair .
	manualset3
115179	4	402526	13	NULL	NULL	0	NULL	physiological processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MMPs play an essential role in several normal physiological processes including growth , wound healing and tissue repair .
	manualset3
115180	5	402526	13	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MMPs play an essential role in several normal physiological processes including growth , wound healing and tissue repair .
	manualset3
115181	6	402526	13	NULL	NULL	0	NULL	wound healing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MMPs play an essential role in several normal physiological processes including growth , wound healing and tissue repair .
	manualset3
115182	7	402526	13	NULL	NULL	0	NULL	tissue repair	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MMPs play an essential role in several normal physiological processes including growth , wound healing and tissue repair .
	manualset3
115183	1	402527	13	NULL	NULL	0	NULL	MNP @ Lectins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	MNP @ Lectins were then applied to human serum , saliva , and urine and the recovered proteins were digested with trypsin and analyzed by nano-HPLC MALDI-TOF/TOF .
	manualset3
115184	2	402527	13	NULL	NULL	0	NULL	human serum 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	MNP @ Lectins were then applied to human serum , saliva , and urine and the recovered proteins were digested with trypsin and analyzed by nano-HPLC MALDI-TOF/TOF .
	manualset3
115185	3	402527	13	NULL	NULL	0	NULL	saliva	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	MNP @ Lectins were then applied to human serum , saliva , and urine and the recovered proteins were digested with trypsin and analyzed by nano-HPLC MALDI-TOF/TOF .
	manualset3
115186	4	402527	13	NULL	NULL	0	NULL	urine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	MNP @ Lectins were then applied to human serum , saliva , and urine and the recovered proteins were digested with trypsin and analyzed by nano-HPLC MALDI-TOF/TOF .
	manualset3
115187	5	402527	13	NULL	NULL	0	NULL	proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	MNP @ Lectins were then applied to human serum , saliva , and urine and the recovered proteins were digested with trypsin and analyzed by nano-HPLC MALDI-TOF/TOF .
	manualset3
115190	6	402527	13	NULL	NULL	0	NULL	trypsin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	MNP @ Lectins were then applied to human serum , saliva , and urine and the recovered proteins were digested with trypsin and analyzed by nano-HPLC MALDI-TOF/TOF .
	manualset3
115191	7	402527	13	NULL	NULL	0	NULL	nano-HPLC MALDI-TOF/TOF	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	MNP @ Lectins were then applied to human serum , saliva , and urine and the recovered proteins were digested with trypsin and analyzed by nano-HPLC MALDI-TOF/TOF .
	manualset3
115192	1	402528	13	NULL	NULL	0	NULL	MNPs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	MNPs have been tested for applications such as targeted drug delivery and controlled drug release and are clinically used as a contrast agent for MRI .
	manualset3
115195	2	402528	13	NULL	NULL	0	NULL	applications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MNPs have been tested for applications such as targeted drug delivery and controlled drug release and are clinically used as a contrast agent for MRI .
	manualset3
115196	3	402528	13	NULL	NULL	0	NULL	drug delivery	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MNPs have been tested for applications such as targeted drug delivery and controlled drug release and are clinically used as a contrast agent for MRI .
	manualset3
115197	4	402528	13	NULL	NULL	0	NULL	drug release	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MNPs have been tested for applications such as targeted drug delivery and controlled drug release and are clinically used as a contrast agent for MRI .
	manualset3
115198	5	402528	13	NULL	NULL	0	NULL	contrast agent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	MNPs have been tested for applications such as targeted drug delivery and controlled drug release and are clinically used as a contrast agent for MRI .
	manualset3
115200	6	402528	13	NULL	NULL	0	NULL	MRI	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	MNPs have been tested for applications such as targeted drug delivery and controlled drug release and are clinically used as a contrast agent for MRI .
	manualset3
115207	1	402529	13	NULL	NULL	0	NULL	MPhi	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	MPhi of chronic and granulomatous inflammation and in tissues that undergo strong antigenic stimulation were strongly positive for TRACP , more so with mab220 than with mab9C5 .
	manualset3
115208	2	402529	13	NULL	NULL	0	NULL	chronic inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MPhi of chronic and granulomatous inflammation and in tissues that undergo strong antigenic stimulation were strongly positive for TRACP , more so with mab220 than with mab9C5 .
	manualset3
115209	3	402529	13	NULL	NULL	0	NULL	granulomatous inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MPhi of chronic and granulomatous inflammation and in tissues that undergo strong antigenic stimulation were strongly positive for TRACP , more so with mab220 than with mab9C5 .
	manualset3
115210	4	402529	13	NULL	NULL	0	NULL	tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	MPhi of chronic and granulomatous inflammation and in tissues that undergo strong antigenic stimulation were strongly positive for TRACP , more so with mab220 than with mab9C5 .
	manualset3
115211	5	402529	13	NULL	NULL	0	NULL	antigenic stimulation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MPhi of chronic and granulomatous inflammation and in tissues that undergo strong antigenic stimulation were strongly positive for TRACP , more so with mab220 than with mab9C5 .
	manualset3
115212	6	402529	13	NULL	NULL	0	NULL	TRACP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	MPhi of chronic and granulomatous inflammation and in tissues that undergo strong antigenic stimulation were strongly positive for TRACP , more so with mab220 than with mab9C5 .
	manualset3
115214	7	402529	13	NULL	NULL	0	NULL	mab220	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	MPhi of chronic and granulomatous inflammation and in tissues that undergo strong antigenic stimulation were strongly positive for TRACP , more so with mab220 than with mab9C5 .
	manualset3
115215	8	402529	13	NULL	NULL	0	NULL	mab9C5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	MPhi of chronic and granulomatous inflammation and in tissues that undergo strong antigenic stimulation were strongly positive for TRACP , more so with mab220 than with mab9C5 .
	manualset3
115216	1	402530	13	NULL	NULL	0	NULL	MR imaging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	MR imaging of the peritoneum and abdominal wall .
	manualset3
115218	2	402530	13	NULL	NULL	0	NULL	peritoneum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	MR imaging of the peritoneum and abdominal wall .
	manualset3
115219	3	402530	13	NULL	NULL	0	NULL	abdominal wall	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	MR imaging of the peritoneum and abdominal wall .
	manualset3
103986	1	402531	5	NULL	NULL	0	NULL	MR imaging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	MR imaging showed a marginal high-intensity area along the aortic wall , while CT showed a nonopacified crescentic area along the aortic wall .
	manualset3
103987	2	402531	5	NULL	NULL	0	NULL	marginal high-intensity area	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	MR imaging showed a marginal high-intensity area along the aortic wall , while CT showed a nonopacified crescentic area along the aortic wall .
	manualset3
103988	3	402531	5	NULL	NULL	0	NULL	aortic wall	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	MR imaging showed a marginal high-intensity area along the aortic wall , while CT showed a nonopacified crescentic area along the aortic wall .
	manualset3
103989	4	402531	5	NULL	NULL	0	NULL	CT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	MR imaging showed a marginal high-intensity area along the aortic wall , while CT showed a nonopacified crescentic area along the aortic wall .
	manualset3
103990	5	402531	5	NULL	NULL	0	NULL	nonopacified crescentic area	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	MR imaging showed a marginal high-intensity area along the aortic wall , while CT showed a nonopacified crescentic area along the aortic wall .
	manualset3
103991	6	402531	5	NULL	NULL	0	NULL	aortic wall	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	MR imaging showed a marginal high-intensity area along the aortic wall , while CT showed a nonopacified crescentic area along the aortic wall .
	manualset3
103992	1	402532	5	NULL	NULL	0	NULL	MR	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	MR in the diagnosis of bone tumors .
	manualset3
103993	2	402532	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	MR in the diagnosis of bone tumors .
	manualset3
103994	3	402532	5	NULL	NULL	0	NULL	bone tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MR in the diagnosis of bone tumors .
	manualset3
103995	1	402533	5	NULL	NULL	0	NULL	MRI analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	MRI analysis were performed to detect segmental atrophy .
	manualset3
103996	2	402533	5	NULL	NULL	0	NULL	segmental atrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MRI analysis were performed to detect segmental atrophy .
	manualset3
103997	1	402534	5	NULL	NULL	NULL	NULL	MRI findings 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	MRI and neurological findings in macrocephaly-cutis marmorata telangiectatica congenita syndrome : report of ten cases and review of the literature : We describe the clinical history and magnetic resonance imaging ( MRI ) findings in 10 children with the Macrocephaly-Cutis Marmorata Telangiectatica Congenita syndrome ( M-CMTC -- MIM 602501 ) .
	manualset3
103998	2	402534	5	NULL	NULL	0	NULL	neurological findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MRI and neurological findings in macrocephaly-cutis marmorata telangiectatica congenita syndrome : report of ten cases and review of the literature : We describe the clinical history and magnetic resonance imaging ( MRI ) findings in 10 children with the Macrocephaly-Cutis Marmorata Telangiectatica Congenita syndrome ( M-CMTC -- MIM 602501 ) .
	manualset3
103999	3	402534	5	NULL	NULL	0	NULL	macrocephaly-cutis marmorata telangiectatica congenita syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	MRI and neurological findings in macrocephaly-cutis marmorata telangiectatica congenita syndrome : report of ten cases and review of the literature : We describe the clinical history and magnetic resonance imaging ( MRI ) findings in 10 children with the Macrocephaly-Cutis Marmorata Telangiectatica Congenita syndrome ( M-CMTC -- MIM 602501 ) .
	manualset3
104000	4	402534	5	NULL	NULL	0	NULL	report 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	MRI and neurological findings in macrocephaly-cutis marmorata telangiectatica congenita syndrome : report of ten cases and review of the literature : We describe the clinical history and magnetic resonance imaging ( MRI ) findings in 10 children with the Macrocephaly-Cutis Marmorata Telangiectatica Congenita syndrome ( M-CMTC -- MIM 602501 ) .
	manualset3
104001	5	402534	5	NULL	NULL	0	NULL	ten cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	MRI and neurological findings in macrocephaly-cutis marmorata telangiectatica congenita syndrome : report of ten cases and review of the literature : We describe the clinical history and magnetic resonance imaging ( MRI ) findings in 10 children with the Macrocephaly-Cutis Marmorata Telangiectatica Congenita syndrome ( M-CMTC -- MIM 602501 ) .
	manualset3
104002	6	402534	5	NULL	NULL	0	NULL	review 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	MRI and neurological findings in macrocephaly-cutis marmorata telangiectatica congenita syndrome : report of ten cases and review of the literature : We describe the clinical history and magnetic resonance imaging ( MRI ) findings in 10 children with the Macrocephaly-Cutis Marmorata Telangiectatica Congenita syndrome ( M-CMTC -- MIM 602501 ) .
	manualset3
104003	7	402534	5	NULL	NULL	0	NULL	literature 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	MRI and neurological findings in macrocephaly-cutis marmorata telangiectatica congenita syndrome : report of ten cases and review of the literature : We describe the clinical history and magnetic resonance imaging ( MRI ) findings in 10 children with the Macrocephaly-Cutis Marmorata Telangiectatica Congenita syndrome ( M-CMTC -- MIM 602501 ) .
	manualset3
104004	8	402534	5	NULL	NULL	0	NULL	describe 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MRI and neurological findings in macrocephaly-cutis marmorata telangiectatica congenita syndrome : report of ten cases and review of the literature : We describe the clinical history and magnetic resonance imaging ( MRI ) findings in 10 children with the Macrocephaly-Cutis Marmorata Telangiectatica Congenita syndrome ( M-CMTC -- MIM 602501 ) .
	manualset3
104005	9	402534	5	NULL	NULL	0	NULL	clinical history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MRI and neurological findings in macrocephaly-cutis marmorata telangiectatica congenita syndrome : report of ten cases and review of the literature : We describe the clinical history and magnetic resonance imaging ( MRI ) findings in 10 children with the Macrocephaly-Cutis Marmorata Telangiectatica Congenita syndrome ( M-CMTC -- MIM 602501 ) .
	manualset3
104006	10	402534	5	NULL	NULL	NULL	NULL	magnetic resonance imaging ( MRI ) findings	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	MRI and neurological findings in macrocephaly-cutis marmorata telangiectatica congenita syndrome : report of ten cases and review of the literature : We describe the clinical history and magnetic resonance imaging ( MRI ) findings in 10 children with the Macrocephaly-Cutis Marmorata Telangiectatica Congenita syndrome ( M-CMTC -- MIM 602501 ) .
	manualset3
104007	11	402534	5	NULL	NULL	0	NULL	10 children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	MRI and neurological findings in macrocephaly-cutis marmorata telangiectatica congenita syndrome : report of ten cases and review of the literature : We describe the clinical history and magnetic resonance imaging ( MRI ) findings in 10 children with the Macrocephaly-Cutis Marmorata Telangiectatica Congenita syndrome ( M-CMTC -- MIM 602501 ) .
	manualset3
104008	12	402534	5	NULL	NULL	0	NULL	Macrocephaly-Cutis Marmorata Telangiectatica Congenita syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	MRI and neurological findings in macrocephaly-cutis marmorata telangiectatica congenita syndrome : report of ten cases and review of the literature : We describe the clinical history and magnetic resonance imaging ( MRI ) findings in 10 children with the Macrocephaly-Cutis Marmorata Telangiectatica Congenita syndrome ( M-CMTC -- MIM 602501 ) .
	manualset3
104009	13	402534	5	NULL	NULL	0	NULL	 M-CMTC -- MIM 602501	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	MRI and neurological findings in macrocephaly-cutis marmorata telangiectatica congenita syndrome : report of ten cases and review of the literature : We describe the clinical history and magnetic resonance imaging ( MRI ) findings in 10 children with the Macrocephaly-Cutis Marmorata Telangiectatica Congenita syndrome ( M-CMTC -- MIM 602501 ) .
	manualset3
104010	1	402535	5	NULL	NULL	0	NULL	MRI infarcts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MRI infarcts , ventricular and sulcal widening , and white matter score were strongly associated with carotid intimal-medial thickness ( IMT ) and stenosis degree after adjustment for age and sex ( all P & lt ; 0 .
	manualset3
104011	2	402535	5	NULL	NULL	0	NULL	ventricular and sulcal widening	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MRI infarcts , ventricular and sulcal widening , and white matter score were strongly associated with carotid intimal-medial thickness ( IMT ) and stenosis degree after adjustment for age and sex ( all P & lt ; 0 .
	manualset3
104012	3	402535	5	NULL	NULL	0	NULL	white matter score	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	MRI infarcts , ventricular and sulcal widening , and white matter score were strongly associated with carotid intimal-medial thickness ( IMT ) and stenosis degree after adjustment for age and sex ( all P & lt ; 0 .
	manualset3
104013	4	402535	5	NULL	NULL	0	NULL	carotid intimal-medial thickness ( IMT )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	MRI infarcts , ventricular and sulcal widening , and white matter score were strongly associated with carotid intimal-medial thickness ( IMT ) and stenosis degree after adjustment for age and sex ( all P & lt ; 0 .
	manualset3
104014	5	402535	5	NULL	NULL	0	NULL	stenosis degree 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	MRI infarcts , ventricular and sulcal widening , and white matter score were strongly associated with carotid intimal-medial thickness ( IMT ) and stenosis degree after adjustment for age and sex ( all P & lt ; 0 .
	manualset3
104015	6	402535	5	NULL	NULL	0	NULL	age	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	MRI infarcts , ventricular and sulcal widening , and white matter score were strongly associated with carotid intimal-medial thickness ( IMT ) and stenosis degree after adjustment for age and sex ( all P & lt ; 0 .
	manualset3
104016	7	402535	5	NULL	NULL	0	NULL	sex	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	MRI infarcts , ventricular and sulcal widening , and white matter score were strongly associated with carotid intimal-medial thickness ( IMT ) and stenosis degree after adjustment for age and sex ( all P & lt ; 0 .
	manualset3
104017	8	402535	5	NULL	NULL	0	NULL	P & lt ; 0	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	MRI infarcts , ventricular and sulcal widening , and white matter score were strongly associated with carotid intimal-medial thickness ( IMT ) and stenosis degree after adjustment for age and sex ( all P & lt ; 0 .
	manualset3
104018	1	402536	5	NULL	NULL	0	NULL	MRSA	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA constituted 38 % of all S. aureus isolates in our 25-bed burns unit despite the utilization of a combination of 1 % silver sulfadiazine and 0.2 % chlorhexidine as topical therapy .
	manualset3
104019	2	402536	5	NULL	NULL	0	NULL	38 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA constituted 38 % of all S. aureus isolates in our 25-bed burns unit despite the utilization of a combination of 1 % silver sulfadiazine and 0.2 % chlorhexidine as topical therapy .
	manualset3
104020	3	402536	5	NULL	NULL	0	NULL	S. aureus isolates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA constituted 38 % of all S. aureus isolates in our 25-bed burns unit despite the utilization of a combination of 1 % silver sulfadiazine and 0.2 % chlorhexidine as topical therapy .
	manualset3
104021	4	402536	5	NULL	NULL	0	NULL	25-bed burns unit	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA constituted 38 % of all S. aureus isolates in our 25-bed burns unit despite the utilization of a combination of 1 % silver sulfadiazine and 0.2 % chlorhexidine as topical therapy .
	manualset3
104022	5	402536	5	NULL	NULL	0	NULL	utilization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA constituted 38 % of all S. aureus isolates in our 25-bed burns unit despite the utilization of a combination of 1 % silver sulfadiazine and 0.2 % chlorhexidine as topical therapy .
	manualset3
104023	6	402536	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA constituted 38 % of all S. aureus isolates in our 25-bed burns unit despite the utilization of a combination of 1 % silver sulfadiazine and 0.2 % chlorhexidine as topical therapy .
	manualset3
104024	7	402536	5	NULL	NULL	0	NULL	1 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA constituted 38 % of all S. aureus isolates in our 25-bed burns unit despite the utilization of a combination of 1 % silver sulfadiazine and 0.2 % chlorhexidine as topical therapy .
	manualset3
104025	8	402536	5	NULL	NULL	0	NULL	silver sulfadiazine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA constituted 38 % of all S. aureus isolates in our 25-bed burns unit despite the utilization of a combination of 1 % silver sulfadiazine and 0.2 % chlorhexidine as topical therapy .
	manualset3
104026	9	402536	5	NULL	NULL	0	NULL	 0.2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA constituted 38 % of all S. aureus isolates in our 25-bed burns unit despite the utilization of a combination of 1 % silver sulfadiazine and 0.2 % chlorhexidine as topical therapy .
	manualset3
104027	10	402536	5	NULL	NULL	0	NULL	chlorhexidine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA constituted 38 % of all S. aureus isolates in our 25-bed burns unit despite the utilization of a combination of 1 % silver sulfadiazine and 0.2 % chlorhexidine as topical therapy .
	manualset3
104028	11	402536	5	NULL	NULL	0	NULL	topical therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA constituted 38 % of all S. aureus isolates in our 25-bed burns unit despite the utilization of a combination of 1 % silver sulfadiazine and 0.2 % chlorhexidine as topical therapy .
	manualset3
104029	1	402537	5	NULL	NULL	0	NULL	MRSA 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA with ST8 increased in the Netherlands from 1 % in 2002 to 17 % in 2003 .
	manualset3
104030	2	402537	5	NULL	NULL	0	NULL	ST8	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA with ST8 increased in the Netherlands from 1 % in 2002 to 17 % in 2003 .
	manualset3
104031	3	402537	5	NULL	NULL	0	NULL	Netherlands 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA with ST8 increased in the Netherlands from 1 % in 2002 to 17 % in 2003 .
	manualset3
104032	4	402537	5	NULL	NULL	0	NULL	1 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA with ST8 increased in the Netherlands from 1 % in 2002 to 17 % in 2003 .
	manualset3
104033	5	402537	5	NULL	NULL	0	NULL	2002 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA with ST8 increased in the Netherlands from 1 % in 2002 to 17 % in 2003 .
	manualset3
104034	6	402537	5	NULL	NULL	0	NULL	17 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA with ST8 increased in the Netherlands from 1 % in 2002 to 17 % in 2003 .
	manualset3
104035	7	402537	5	NULL	NULL	0	NULL	2003	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	MRSA with ST8 increased in the Netherlands from 1 % in 2002 to 17 % in 2003 .
	manualset3
104036	1	402538	5	NULL	NULL	0	NULL	MULTIPLE MYELOMA	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	MULTIPLE MYELOMA AS A SINGLE LESION .
	manualset3
104037	2	402538	5	NULL	NULL	0	NULL	SINGLE LESION        	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MULTIPLE MYELOMA AS A SINGLE LESION .
	manualset3
104056	1	402539	5	NULL	NULL	0	NULL	CE-MS method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A CE-MS method was developed and validated for the quantitative analysis of negatively charged metabolites by making use of the high mass accuracy and the quantitation capabilities of a TOF mass analyzer in combination with automated feature extraction and database search .
	manualset3
104059	2	402539	5	NULL	NULL	0	NULL	quantitative analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A CE-MS method was developed and validated for the quantitative analysis of negatively charged metabolites by making use of the high mass accuracy and the quantitation capabilities of a TOF mass analyzer in combination with automated feature extraction and database search .
	manualset3
104063	3	402539	5	NULL	NULL	0	NULL	negatively charged metabolites	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	A CE-MS method was developed and validated for the quantitative analysis of negatively charged metabolites by making use of the high mass accuracy and the quantitation capabilities of a TOF mass analyzer in combination with automated feature extraction and database search .
	manualset3
104065	4	402539	5	NULL	NULL	0	NULL	high mass accuracy	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A CE-MS method was developed and validated for the quantitative analysis of negatively charged metabolites by making use of the high mass accuracy and the quantitation capabilities of a TOF mass analyzer in combination with automated feature extraction and database search .
	manualset3
104066	5	402539	5	NULL	NULL	0	NULL	quantitation capabilities	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A CE-MS method was developed and validated for the quantitative analysis of negatively charged metabolites by making use of the high mass accuracy and the quantitation capabilities of a TOF mass analyzer in combination with automated feature extraction and database search .
	manualset3
104067	6	402539	5	NULL	NULL	0	NULL	TOF mass analyzer	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A CE-MS method was developed and validated for the quantitative analysis of negatively charged metabolites by making use of the high mass accuracy and the quantitation capabilities of a TOF mass analyzer in combination with automated feature extraction and database search .
	manualset3
104068	7	402539	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A CE-MS method was developed and validated for the quantitative analysis of negatively charged metabolites by making use of the high mass accuracy and the quantitation capabilities of a TOF mass analyzer in combination with automated feature extraction and database search .
	manualset3
104069	8	402539	5	NULL	NULL	0	NULL	automated feature extraction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A CE-MS method was developed and validated for the quantitative analysis of negatively charged metabolites by making use of the high mass accuracy and the quantitation capabilities of a TOF mass analyzer in combination with automated feature extraction and database search .
	manualset3
104070	9	402539	5	NULL	NULL	0	NULL	database search	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A CE-MS method was developed and validated for the quantitative analysis of negatively charged metabolites by making use of the high mass accuracy and the quantitation capabilities of a TOF mass analyzer in combination with automated feature extraction and database search .
	manualset3
104073	1	402540	5	NULL	NULL	0	NULL	Macedonia 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Macedonia is an endemic region of cattle as well as of sheep and goat piroplasmosis In cattle , Theileria orientalis ( = T. buffeli ? )
	manualset3
104074	2	402540	5	NULL	NULL	0	NULL	endemic region	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Macedonia is an endemic region of cattle as well as of sheep and goat piroplasmosis In cattle , Theileria orientalis ( = T. buffeli ? )
	manualset3
104075	3	402540	5	NULL	NULL	NULL	NULL	cattle piroplasmosis 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Macedonia is an endemic region of cattle as well as of sheep and goat piroplasmosis In cattle , Theileria orientalis ( = T. buffeli ? )
	manualset3
104077	4	402540	5	NULL	NULL	NULL	NULL	sheep piroplasmosis 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Macedonia is an endemic region of cattle as well as of sheep and goat piroplasmosis In cattle , Theileria orientalis ( = T. buffeli ? )
	manualset3
104081	5	402540	5	NULL	NULL	0	NULL	goat piroplasmosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Macedonia is an endemic region of cattle as well as of sheep and goat piroplasmosis In cattle , Theileria orientalis ( = T. buffeli ? )
	manualset3
104084	6	402540	5	NULL	NULL	0	NULL	cattle 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Macedonia is an endemic region of cattle as well as of sheep and goat piroplasmosis In cattle , Theileria orientalis ( = T. buffeli ? )
	manualset3
104085	7	402540	5	NULL	NULL	0	NULL	Theileria orientalis ( = T. buffeli ? )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Macedonia is an endemic region of cattle as well as of sheep and goat piroplasmosis In cattle , Theileria orientalis ( = T. buffeli ? )
	manualset3
104086	2	402541	5	NULL	NULL	NULL	NULL	ultrasound-assisted extraction ( USAE )	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Maceration , ultrasound-assisted ( USAE ) and microwave assisted extraction ( MAE ) were applied .
	manualset3
104087	3	402541	5	NULL	NULL	0	NULL	microwave assisted extraction ( MAE )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Maceration , ultrasound-assisted ( USAE ) and microwave assisted extraction ( MAE ) were applied .
	manualset3
104088	1	402541	5	NULL	NULL	NULL	NULL	Maceration 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Maceration , ultrasound-assisted ( USAE ) and microwave assisted extraction ( MAE ) were applied .
	manualset3
104091	1	402542	5	NULL	NULL	0	NULL	Machakos Project Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Machakos Project Studies : Agents affecting health of mother and child in a rural area of Kenya .
	manualset3
104092	2	402542	5	NULL	NULL	0	NULL	Agents 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Machakos Project Studies : Agents affecting health of mother and child in a rural area of Kenya .
	manualset3
104093	3	402542	5	NULL	NULL	0	NULL	health 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Machakos Project Studies : Agents affecting health of mother and child in a rural area of Kenya .
	manualset3
104095	4	402542	5	NULL	NULL	0	NULL	mother 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Machakos Project Studies : Agents affecting health of mother and child in a rural area of Kenya .
	manualset3
104097	5	402542	5	NULL	NULL	0	NULL	child 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Machakos Project Studies : Agents affecting health of mother and child in a rural area of Kenya .
	manualset3
104098	6	402542	5	NULL	NULL	0	NULL	rural area	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Machakos Project Studies : Agents affecting health of mother and child in a rural area of Kenya .
	manualset3
104100	7	402542	5	NULL	NULL	0	NULL	Kenya 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Machakos Project Studies : Agents affecting health of mother and child in a rural area of Kenya .
	manualset3
104103	1	402543	5	NULL	NULL	0	NULL	Macromolecular adducts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Macromolecular adducts caused by environmental chemicals .
	manualset3
104108	2	402543	5	NULL	NULL	0	NULL	environmental chemicals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Macromolecular adducts caused by environmental chemicals .
	manualset3
104111	1	402544	5	NULL	NULL	0	NULL	Macrophage migration inhibitory factor ( MIF )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Macrophage migration inhibitory factor ( MIF ) , a proinflammatory mediator , has been shown to be elevated following heart surgery in adults and may be associated with several postoperative complications , including cardiac and pulmonary dysfunction .
	manualset3
104113	2	402544	5	NULL	NULL	0	NULL	proinflammatory mediator	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Macrophage migration inhibitory factor ( MIF ) , a proinflammatory mediator , has been shown to be elevated following heart surgery in adults and may be associated with several postoperative complications , including cardiac and pulmonary dysfunction .
	manualset3
104115	3	402544	5	NULL	NULL	0	NULL	heart surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Macrophage migration inhibitory factor ( MIF ) , a proinflammatory mediator , has been shown to be elevated following heart surgery in adults and may be associated with several postoperative complications , including cardiac and pulmonary dysfunction .
	manualset3
104116	4	402544	5	NULL	NULL	0	NULL	adults 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Macrophage migration inhibitory factor ( MIF ) , a proinflammatory mediator , has been shown to be elevated following heart surgery in adults and may be associated with several postoperative complications , including cardiac and pulmonary dysfunction .
	manualset3
104117	5	402544	5	NULL	NULL	0	NULL	several postoperative complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Macrophage migration inhibitory factor ( MIF ) , a proinflammatory mediator , has been shown to be elevated following heart surgery in adults and may be associated with several postoperative complications , including cardiac and pulmonary dysfunction .
	manualset3
104118	6	402544	5	NULL	NULL	0	NULL	cardiac dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Macrophage migration inhibitory factor ( MIF ) , a proinflammatory mediator , has been shown to be elevated following heart surgery in adults and may be associated with several postoperative complications , including cardiac and pulmonary dysfunction .
	manualset3
104119	7	402544	5	NULL	NULL	0	NULL	pulmonary dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Macrophage migration inhibitory factor ( MIF ) , a proinflammatory mediator , has been shown to be elevated following heart surgery in adults and may be associated with several postoperative complications , including cardiac and pulmonary dysfunction .
	manualset3
104120	1	402545	5	NULL	NULL	0	NULL	Macrophages 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Macrophages at an inflammatory site release massive amounts of proteolytic enzymes , including lysosomal cysteine proteases , which colocalize with their circulating , tight-binding inhibitors ( cystatins , kininogens ) , so modifying the protease/antiprotease equilibrium in favor of enhanced proteolysis .
	manualset3
104121	2	402545	5	NULL	NULL	0	NULL	inflammatory site	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Macrophages at an inflammatory site release massive amounts of proteolytic enzymes , including lysosomal cysteine proteases , which colocalize with their circulating , tight-binding inhibitors ( cystatins , kininogens ) , so modifying the protease/antiprotease equilibrium in favor of enhanced proteolysis .
	manualset3
104122	3	402545	5	NULL	NULL	0	NULL	massive amounts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Macrophages at an inflammatory site release massive amounts of proteolytic enzymes , including lysosomal cysteine proteases , which colocalize with their circulating , tight-binding inhibitors ( cystatins , kininogens ) , so modifying the protease/antiprotease equilibrium in favor of enhanced proteolysis .
	manualset3
104123	4	402545	5	NULL	NULL	0	NULL	proteolytic enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Macrophages at an inflammatory site release massive amounts of proteolytic enzymes , including lysosomal cysteine proteases , which colocalize with their circulating , tight-binding inhibitors ( cystatins , kininogens ) , so modifying the protease/antiprotease equilibrium in favor of enhanced proteolysis .
	manualset3
104124	5	402545	5	NULL	NULL	0	NULL	lysosomal cysteine proteases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Macrophages at an inflammatory site release massive amounts of proteolytic enzymes , including lysosomal cysteine proteases , which colocalize with their circulating , tight-binding inhibitors ( cystatins , kininogens ) , so modifying the protease/antiprotease equilibrium in favor of enhanced proteolysis .
	manualset3
104125	6	402545	5	NULL	NULL	0	NULL	circulating , tight-binding inhibitors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Macrophages at an inflammatory site release massive amounts of proteolytic enzymes , including lysosomal cysteine proteases , which colocalize with their circulating , tight-binding inhibitors ( cystatins , kininogens ) , so modifying the protease/antiprotease equilibrium in favor of enhanced proteolysis .
	manualset3
104126	7	402545	5	NULL	NULL	0	NULL	cystatins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Macrophages at an inflammatory site release massive amounts of proteolytic enzymes , including lysosomal cysteine proteases , which colocalize with their circulating , tight-binding inhibitors ( cystatins , kininogens ) , so modifying the protease/antiprotease equilibrium in favor of enhanced proteolysis .
	manualset3
104127	8	402545	5	NULL	NULL	0	NULL	kininogens 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Macrophages at an inflammatory site release massive amounts of proteolytic enzymes , including lysosomal cysteine proteases , which colocalize with their circulating , tight-binding inhibitors ( cystatins , kininogens ) , so modifying the protease/antiprotease equilibrium in favor of enhanced proteolysis .
	manualset3
104128	9	402545	5	NULL	NULL	0	NULL	protease/antiprotease equilibrium	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Macrophages at an inflammatory site release massive amounts of proteolytic enzymes , including lysosomal cysteine proteases , which colocalize with their circulating , tight-binding inhibitors ( cystatins , kininogens ) , so modifying the protease/antiprotease equilibrium in favor of enhanced proteolysis .
	manualset3
104129	10	402545	5	NULL	NULL	0	NULL	enhanced proteolysis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Macrophages at an inflammatory site release massive amounts of proteolytic enzymes , including lysosomal cysteine proteases , which colocalize with their circulating , tight-binding inhibitors ( cystatins , kininogens ) , so modifying the protease/antiprotease equilibrium in favor of enhanced proteolysis .
	manualset3
104130	1	402546	5	NULL	NULL	0	NULL	Macrophages 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Macrophages possess a variety of surface receptors devoted to the recognition of non-self by discriminating between host and pathogen-derived structures .
	manualset3
104131	2	402546	5	NULL	NULL	0	NULL	surface receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Macrophages possess a variety of surface receptors devoted to the recognition of non-self by discriminating between host and pathogen-derived structures .
	manualset3
104132	3	402546	5	NULL	NULL	NULL	NULL	recognition of non-self	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Macrophages possess a variety of surface receptors devoted to the recognition of non-self by discriminating between host and pathogen-derived structures .
	manualset3
104133	4	402546	5	NULL	NULL	0	NULL	host 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Macrophages possess a variety of surface receptors devoted to the recognition of non-self by discriminating between host and pathogen-derived structures .
	manualset3
104134	5	402546	5	NULL	NULL	0	NULL	pathogen-derived structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Macrophages possess a variety of surface receptors devoted to the recognition of non-self by discriminating between host and pathogen-derived structures .
	manualset3
104135	1	402547	5	NULL	NULL	0	NULL	Macrophages 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Macrophages proliferate until an endotoxic shock halts cell growth and they become activated .
	manualset3
104136	2	402547	5	NULL	NULL	0	NULL	endotoxic shock	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Macrophages proliferate until an endotoxic shock halts cell growth and they become activated .
	manualset3
104137	3	402547	5	NULL	NULL	0	NULL	cell growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Macrophages proliferate until an endotoxic shock halts cell growth and they become activated .
	manualset3
104138	1	402548	5	NULL	NULL	0	NULL	Macroscopic studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Macroscopic studies of the liver , lungs , spleen , kidney , and brain were performed .
	manualset3
104139	2	402548	5	NULL	NULL	0	NULL	liver 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Macroscopic studies of the liver , lungs , spleen , kidney , and brain were performed .
	manualset3
104140	3	402548	5	NULL	NULL	0	NULL	lungs 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Macroscopic studies of the liver , lungs , spleen , kidney , and brain were performed .
	manualset3
104141	4	402548	5	NULL	NULL	0	NULL	spleen 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Macroscopic studies of the liver , lungs , spleen , kidney , and brain were performed .
	manualset3
104142	5	402548	5	NULL	NULL	0	NULL	kidney 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Macroscopic studies of the liver , lungs , spleen , kidney , and brain were performed .
	manualset3
104143	6	402548	5	NULL	NULL	0	NULL	brain 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Macroscopic studies of the liver , lungs , spleen , kidney , and brain were performed .
	manualset3
104144	1	402549	5	NULL	NULL	0	NULL	intoxication 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Macroscopically the intoxication in ostriches resulted in a severe anasarca of the neck and ventral body .
	manualset3
104145	2	402549	5	NULL	NULL	0	NULL	ostriches 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Macroscopically the intoxication in ostriches resulted in a severe anasarca of the neck and ventral body .
	manualset3
104146	3	402549	5	NULL	NULL	0	NULL	severe anasarca	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Macroscopically the intoxication in ostriches resulted in a severe anasarca of the neck and ventral body .
	manualset3
104147	4	402549	5	NULL	NULL	0	NULL	neck 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Macroscopically the intoxication in ostriches resulted in a severe anasarca of the neck and ventral body .
	manualset3
104148	5	402549	5	NULL	NULL	0	NULL	ventral body	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Macroscopically the intoxication in ostriches resulted in a severe anasarca of the neck and ventral body .
	manualset3
104158	1	402550	5	NULL	NULL	0	NULL	Magnetic field exposure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic field exposure during gestation : pineal and cerebral cortex serotonin in the rat .
	manualset3
104159	2	402550	5	NULL	NULL	0	NULL	gestation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic field exposure during gestation : pineal and cerebral cortex serotonin in the rat .
	manualset3
104160	3	402550	5	NULL	NULL	NULL	NULL	pineal serotonin	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Magnetic field exposure during gestation : pineal and cerebral cortex serotonin in the rat .
	manualset3
104161	4	402550	5	NULL	NULL	0	NULL	cerebral cortex serotonin	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic field exposure during gestation : pineal and cerebral cortex serotonin in the rat .
	manualset3
104164	5	402550	5	NULL	NULL	0	NULL	rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic field exposure during gestation : pineal and cerebral cortex serotonin in the rat .
	manualset3
104166	1	402551	5	NULL	NULL	0	NULL	Magnetic fields ( MF )	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic fields ( MF ) of 50 Hz at 1.2 microT as well as 100 microT cause uncoupling of inhibitory pathways of adenylyl cyclase mediated by melatonin 1a receptor in MF-sensitive MCF-7 cells .
	manualset3
104168	2	402551	5	NULL	NULL	0	NULL	50 Hz	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic fields ( MF ) of 50 Hz at 1.2 microT as well as 100 microT cause uncoupling of inhibitory pathways of adenylyl cyclase mediated by melatonin 1a receptor in MF-sensitive MCF-7 cells .
	manualset3
104171	3	402551	5	NULL	NULL	0	NULL	1.2 microT	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic fields ( MF ) of 50 Hz at 1.2 microT as well as 100 microT cause uncoupling of inhibitory pathways of adenylyl cyclase mediated by melatonin 1a receptor in MF-sensitive MCF-7 cells .
	manualset3
104172	4	402551	5	NULL	NULL	0	NULL	100 microT	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic fields ( MF ) of 50 Hz at 1.2 microT as well as 100 microT cause uncoupling of inhibitory pathways of adenylyl cyclase mediated by melatonin 1a receptor in MF-sensitive MCF-7 cells .
	manualset3
104173	5	402551	5	NULL	NULL	0	NULL	inhibitory pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic fields ( MF ) of 50 Hz at 1.2 microT as well as 100 microT cause uncoupling of inhibitory pathways of adenylyl cyclase mediated by melatonin 1a receptor in MF-sensitive MCF-7 cells .
	manualset3
104174	6	402551	5	NULL	NULL	0	NULL	adenylyl cyclase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic fields ( MF ) of 50 Hz at 1.2 microT as well as 100 microT cause uncoupling of inhibitory pathways of adenylyl cyclase mediated by melatonin 1a receptor in MF-sensitive MCF-7 cells .
	manualset3
104175	7	402551	5	NULL	NULL	0	NULL	melatonin 1a receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic fields ( MF ) of 50 Hz at 1.2 microT as well as 100 microT cause uncoupling of inhibitory pathways of adenylyl cyclase mediated by melatonin 1a receptor in MF-sensitive MCF-7 cells .
	manualset3
104176	8	402551	5	NULL	NULL	0	NULL	MF-sensitive MCF-7 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic fields ( MF ) of 50 Hz at 1.2 microT as well as 100 microT cause uncoupling of inhibitory pathways of adenylyl cyclase mediated by melatonin 1a receptor in MF-sensitive MCF-7 cells .
	manualset3
104177	1	402552	5	NULL	NULL	0	NULL	Magnetic maps	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic maps in animals : a theory comes of age ?
	manualset3
104178	2	402552	5	NULL	NULL	0	NULL	animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic maps in animals : a theory comes of age ?
	manualset3
104179	3	402552	5	NULL	NULL	0	NULL	theory 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic maps in animals : a theory comes of age ?
	manualset3
104180	4	402552	5	NULL	NULL	0	NULL	age	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic maps in animals : a theory comes of age ?
	manualset3
104181	1	402553	5	NULL	NULL	0	NULL	Magnetic resonance electrical impedance tomography ( MREIT )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic resonance electrical impedance tomography ( MREIT ) : simulation study of J-substitution algorithm .
	manualset3
104182	2	402553	5	NULL	NULL	0	NULL	simulation study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic resonance electrical impedance tomography ( MREIT ) : simulation study of J-substitution algorithm .
	manualset3
104183	3	402553	5	NULL	NULL	0	NULL	J-substitution algorithm	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic resonance electrical impedance tomography ( MREIT ) : simulation study of J-substitution algorithm .
	manualset3
104187	1	402554	5	NULL	NULL	0	NULL	Magnetic resonance imaging-based assessment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic resonance imaging-based assessment of cartilage loss in severe osteoarthritis : accuracy , precision , and diagnostic value .
	manualset3
104189	2	402554	5	NULL	NULL	0	NULL	cartilage loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic resonance imaging-based assessment of cartilage loss in severe osteoarthritis : accuracy , precision , and diagnostic value .
	manualset3
104190	3	402554	5	NULL	NULL	0	NULL	severe osteoarthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic resonance imaging-based assessment of cartilage loss in severe osteoarthritis : accuracy , precision , and diagnostic value .
	manualset3
104191	4	402554	5	NULL	NULL	0	NULL	accuracy 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic resonance imaging-based assessment of cartilage loss in severe osteoarthritis : accuracy , precision , and diagnostic value .
	manualset3
104192	5	402554	5	NULL	NULL	0	NULL	precision 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic resonance imaging-based assessment of cartilage loss in severe osteoarthritis : accuracy , precision , and diagnostic value .
	manualset3
104193	6	402554	5	NULL	NULL	0	NULL	diagnostic value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic resonance imaging-based assessment of cartilage loss in severe osteoarthritis : accuracy , precision , and diagnostic value .
	manualset3
104194	1	402555	5	NULL	NULL	0	NULL	Magnetic resonance imaging ( MRI ) 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic resonance imaging ( MRI ) revealed localized abnormalities of calf muscles .
	manualset3
104195	2	402555	5	NULL	NULL	0	NULL	localized abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic resonance imaging ( MRI ) revealed localized abnormalities of calf muscles .
	manualset3
104196	3	402555	5	NULL	NULL	0	NULL	calf muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic resonance imaging ( MRI ) revealed localized abnormalities of calf muscles .
	manualset3
104198	1	402556	5	NULL	NULL	0	NULL	Magnetic resonance imaging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic resonance imaging now has been shown to be the most sensitive imaging technique available for the detection of bone metastases .
	manualset3
104200	2	402556	5	NULL	NULL	0	NULL	 sensitive imaging technique	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic resonance imaging now has been shown to be the most sensitive imaging technique available for the detection of bone metastases .
	manualset3
104202	3	402556	5	NULL	NULL	0	NULL	detection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic resonance imaging now has been shown to be the most sensitive imaging technique available for the detection of bone metastases .
	manualset3
104203	4	402556	5	NULL	NULL	0	NULL	bone metastases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic resonance imaging now has been shown to be the most sensitive imaging technique available for the detection of bone metastases .
	manualset3
104244	1	402557	5	NULL	NULL	0	NULL	indications 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Main indications for liver transplantation were a very low initial Quick 's test score and factor V value ( both & lt ; 10 % ) and their inadequate response under substitution therapy .
	manualset3
104245	2	402557	5	NULL	NULL	0	NULL	liver transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Main indications for liver transplantation were a very low initial Quick 's test score and factor V value ( both & lt ; 10 % ) and their inadequate response under substitution therapy .
	manualset3
104246	3	402557	5	NULL	NULL	0	NULL	very low initial Quick 's test score	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Main indications for liver transplantation were a very low initial Quick 's test score and factor V value ( both & lt ; 10 % ) and their inadequate response under substitution therapy .
	manualset3
104247	4	402557	5	NULL	NULL	0	NULL	factor V value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Main indications for liver transplantation were a very low initial Quick 's test score and factor V value ( both & lt ; 10 % ) and their inadequate response under substitution therapy .
	manualset3
104248	5	402557	5	NULL	NULL	0	NULL	 lt ; 10 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Main indications for liver transplantation were a very low initial Quick 's test score and factor V value ( both & lt ; 10 % ) and their inadequate response under substitution therapy .
	manualset3
104249	6	402557	5	NULL	NULL	0	NULL	inadequate response 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Main indications for liver transplantation were a very low initial Quick 's test score and factor V value ( both & lt ; 10 % ) and their inadequate response under substitution therapy .
	manualset3
104250	7	402557	5	NULL	NULL	0	NULL	substitution therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Main indications for liver transplantation were a very low initial Quick 's test score and factor V value ( both & lt ; 10 % ) and their inadequate response under substitution therapy .
	manualset3
104251	1	402558	5	NULL	NULL	0	NULL	A Canada Fit for Children	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A Canada Fit for Children is an essential tool for child and youth health care givers .
	manualset3
104252	2	402558	5	NULL	NULL	0	NULL	essential tool	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A Canada Fit for Children is an essential tool for child and youth health care givers .
	manualset3
104254	3	402558	5	NULL	NULL	0	NULL	child health care givers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A Canada Fit for Children is an essential tool for child and youth health care givers .
	manualset3
104256	4	402558	5	NULL	NULL	0	NULL	youth health care givers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A Canada Fit for Children is an essential tool for child and youth health care givers .
	manualset3
104257	1	402559	5	NULL	NULL	0	NULL	Maintenance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Maintenance of fibrin solubility by plasma fibronectin .
	manualset3
104258	2	402559	5	NULL	NULL	0	NULL	fibrin solubility	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Maintenance of fibrin solubility by plasma fibronectin .
	manualset3
104260	3	402559	5	NULL	NULL	0	NULL	plasma fibronectin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Maintenance of fibrin solubility by plasma fibronectin .
	manualset3
104263	1	402560	5	NULL	NULL	NULL	NULL	Maintenance of hormonal activity	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Maintenance of hormonal activity was assessed by detection of gastrin levels during the first 3 months in culture .
	manualset3
104264	2	402560	5	NULL	NULL	0	NULL	detection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Maintenance of hormonal activity was assessed by detection of gastrin levels during the first 3 months in culture .
	manualset3
104265	3	402560	5	NULL	NULL	0	NULL	gastrin levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Maintenance of hormonal activity was assessed by detection of gastrin levels during the first 3 months in culture .
	manualset3
104266	4	402560	5	NULL	NULL	0	NULL	first 3 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Maintenance of hormonal activity was assessed by detection of gastrin levels during the first 3 months in culture .
	manualset3
104267	5	402560	5	NULL	NULL	0	NULL	culture 	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Maintenance of hormonal activity was assessed by detection of gastrin levels during the first 3 months in culture .
	manualset3
104268	1	402561	5	NULL	NULL	0	NULL	Maintenance therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Maintenance therapy consisted of 1.2-1 .6 mg/kg/day of cytosine arabinoside , twice a week or 2 mg/kg/day of 6 MP orally .
	manualset3
104269	2	402561	5	NULL	NULL	0	NULL	1.2-1 .6 mg/kg/day 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Maintenance therapy consisted of 1.2-1 .6 mg/kg/day of cytosine arabinoside , twice a week or 2 mg/kg/day of 6 MP orally .
	manualset3
104273	3	402561	5	NULL	NULL	0	NULL	cytosine arabinoside	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Maintenance therapy consisted of 1.2-1 .6 mg/kg/day of cytosine arabinoside , twice a week or 2 mg/kg/day of 6 MP orally .
	manualset3
104274	4	402561	5	NULL	NULL	NULL	NULL	twice a week	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Maintenance therapy consisted of 1.2-1 .6 mg/kg/day of cytosine arabinoside , twice a week or 2 mg/kg/day of 6 MP orally .
	manualset3
104275	5	402561	5	NULL	NULL	0	NULL	2 mg/kg/day	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Maintenance therapy consisted of 1.2-1 .6 mg/kg/day of cytosine arabinoside , twice a week or 2 mg/kg/day of 6 MP orally .
	manualset3
104276	6	402561	5	NULL	NULL	0	NULL	6 MP	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Maintenance therapy consisted of 1.2-1 .6 mg/kg/day of cytosine arabinoside , twice a week or 2 mg/kg/day of 6 MP orally .
	manualset3
104277	1	402562	5	NULL	NULL	0	NULL	Maintenance treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Maintenance treatment has been demonstrated to be an effective treatment for opioid addiction but still lacks quality of life specific measures to measure the maintenance program effects and until now there have been only few attempts to assess the impact of opioid dependence and its treatment on the drug-addicted patients ' quality of life .
	manualset3
104278	2	402562	5	NULL	NULL	0	NULL	effective treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Maintenance treatment has been demonstrated to be an effective treatment for opioid addiction but still lacks quality of life specific measures to measure the maintenance program effects and until now there have been only few attempts to assess the impact of opioid dependence and its treatment on the drug-addicted patients ' quality of life .
	manualset3
104279	3	402562	5	NULL	NULL	0	NULL	opioid addiction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Maintenance treatment has been demonstrated to be an effective treatment for opioid addiction but still lacks quality of life specific measures to measure the maintenance program effects and until now there have been only few attempts to assess the impact of opioid dependence and its treatment on the drug-addicted patients ' quality of life .
	manualset3
104280	4	402562	5	NULL	NULL	0	NULL	quality of life	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Maintenance treatment has been demonstrated to be an effective treatment for opioid addiction but still lacks quality of life specific measures to measure the maintenance program effects and until now there have been only few attempts to assess the impact of opioid dependence and its treatment on the drug-addicted patients ' quality of life .
	manualset3
104281	5	402562	5	NULL	NULL	0	NULL	specific measures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Maintenance treatment has been demonstrated to be an effective treatment for opioid addiction but still lacks quality of life specific measures to measure the maintenance program effects and until now there have been only few attempts to assess the impact of opioid dependence and its treatment on the drug-addicted patients ' quality of life .
	manualset3
104283	7	402562	5	NULL	NULL	0	NULL	maintenance program effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Maintenance treatment has been demonstrated to be an effective treatment for opioid addiction but still lacks quality of life specific measures to measure the maintenance program effects and until now there have been only few attempts to assess the impact of opioid dependence and its treatment on the drug-addicted patients ' quality of life .
	manualset3
104284	8	402562	5	NULL	NULL	NULL	NULL	attempts	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Maintenance treatment has been demonstrated to be an effective treatment for opioid addiction but still lacks quality of life specific measures to measure the maintenance program effects and until now there have been only few attempts to assess the impact of opioid dependence and its treatment on the drug-addicted patients ' quality of life .
	manualset3
104285	9	402562	5	NULL	NULL	0	NULL	impact 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Maintenance treatment has been demonstrated to be an effective treatment for opioid addiction but still lacks quality of life specific measures to measure the maintenance program effects and until now there have been only few attempts to assess the impact of opioid dependence and its treatment on the drug-addicted patients ' quality of life .
	manualset3
104286	10	402562	5	NULL	NULL	0	NULL	opioid dependence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Maintenance treatment has been demonstrated to be an effective treatment for opioid addiction but still lacks quality of life specific measures to measure the maintenance program effects and until now there have been only few attempts to assess the impact of opioid dependence and its treatment on the drug-addicted patients ' quality of life .
	manualset3
104287	11	402562	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Maintenance treatment has been demonstrated to be an effective treatment for opioid addiction but still lacks quality of life specific measures to measure the maintenance program effects and until now there have been only few attempts to assess the impact of opioid dependence and its treatment on the drug-addicted patients ' quality of life .
	manualset3
104288	12	402562	5	NULL	NULL	0	NULL	drug-addicted patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Maintenance treatment has been demonstrated to be an effective treatment for opioid addiction but still lacks quality of life specific measures to measure the maintenance program effects and until now there have been only few attempts to assess the impact of opioid dependence and its treatment on the drug-addicted patients ' quality of life .
	manualset3
104289	13	402562	5	NULL	NULL	0	NULL	quality of life	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Maintenance treatment has been demonstrated to be an effective treatment for opioid addiction but still lacks quality of life specific measures to measure the maintenance program effects and until now there have been only few attempts to assess the impact of opioid dependence and its treatment on the drug-addicted patients ' quality of life .
	manualset3
104290	1	402563	5	NULL	NULL	0	NULL	Major complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Major complications in the post-operative course were the leakage of anastomosis and respiratory failure .
	manualset3
104291	2	402563	5	NULL	NULL	0	NULL	post-operative course 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Major complications in the post-operative course were the leakage of anastomosis and respiratory failure .
	manualset3
104292	3	402563	5	NULL	NULL	0	NULL	leakage of anastomosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Major complications in the post-operative course were the leakage of anastomosis and respiratory failure .
	manualset3
104293	4	402563	5	NULL	NULL	0	NULL	respiratory failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Major complications in the post-operative course were the leakage of anastomosis and respiratory failure .
	manualset3
104294	1	402564	5	NULL	NULL	0	NULL	Major histocompatibility complex molecules ( HLA )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Major histocompatibility complex molecules ( HLA ) , the co-stimulatory molecule B7 and the intercellular adhesion molecule 1 ( ICAM-1 ) are key molecules involved in T cell-mediated immune surveillance .
	manualset3
104295	2	402564	5	NULL	NULL	0	NULL	co-stimulatory molecule B7	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Major histocompatibility complex molecules ( HLA ) , the co-stimulatory molecule B7 and the intercellular adhesion molecule 1 ( ICAM-1 ) are key molecules involved in T cell-mediated immune surveillance .
	manualset3
104296	3	402564	5	NULL	NULL	0	NULL	intercellular adhesion molecule 1 ( ICAM-1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Major histocompatibility complex molecules ( HLA ) , the co-stimulatory molecule B7 and the intercellular adhesion molecule 1 ( ICAM-1 ) are key molecules involved in T cell-mediated immune surveillance .
	manualset3
104297	4	402564	5	NULL	NULL	0	NULL	key molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Major histocompatibility complex molecules ( HLA ) , the co-stimulatory molecule B7 and the intercellular adhesion molecule 1 ( ICAM-1 ) are key molecules involved in T cell-mediated immune surveillance .
	manualset3
104298	5	402564	5	NULL	NULL	0	NULL	T cell-mediated immune surveillance	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Major histocompatibility complex molecules ( HLA ) , the co-stimulatory molecule B7 and the intercellular adhesion molecule 1 ( ICAM-1 ) are key molecules involved in T cell-mediated immune surveillance .
	manualset3
104299	1	402565	5	NULL	NULL	0	NULL	advances 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Major new advances in biomedical medicine , especially in immunology and molecular biology , are gradually being applied to the evaluation of bronchoalveolar lavage , thus further extending the efficacy of this procedure .
	manualset3
104300	2	402565	5	NULL	NULL	0	NULL	biomedical medicine	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Major new advances in biomedical medicine , especially in immunology and molecular biology , are gradually being applied to the evaluation of bronchoalveolar lavage , thus further extending the efficacy of this procedure .
	manualset3
104301	3	402565	5	NULL	NULL	0	NULL	immunology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Major new advances in biomedical medicine , especially in immunology and molecular biology , are gradually being applied to the evaluation of bronchoalveolar lavage , thus further extending the efficacy of this procedure .
	manualset3
104302	4	402565	5	NULL	NULL	0	NULL	molecular biology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Major new advances in biomedical medicine , especially in immunology and molecular biology , are gradually being applied to the evaluation of bronchoalveolar lavage , thus further extending the efficacy of this procedure .
	manualset3
104303	5	402565	5	NULL	NULL	0	NULL	evaluation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Major new advances in biomedical medicine , especially in immunology and molecular biology , are gradually being applied to the evaluation of bronchoalveolar lavage , thus further extending the efficacy of this procedure .
	manualset3
104304	6	402565	5	NULL	NULL	0	NULL	bronchoalveolar lavage	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Major new advances in biomedical medicine , especially in immunology and molecular biology , are gradually being applied to the evaluation of bronchoalveolar lavage , thus further extending the efficacy of this procedure .
	manualset3
104305	7	402565	5	NULL	NULL	0	NULL	efficacy 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Major new advances in biomedical medicine , especially in immunology and molecular biology , are gradually being applied to the evaluation of bronchoalveolar lavage , thus further extending the efficacy of this procedure .
	manualset3
104306	8	402565	5	NULL	NULL	0	NULL	procedure 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Major new advances in biomedical medicine , especially in immunology and molecular biology , are gradually being applied to the evaluation of bronchoalveolar lavage , thus further extending the efficacy of this procedure .
	manualset3
104307	1	402566	5	NULL	NULL	NULL	NULL	Major pathways of carbon metabolism	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Major pathways of carbon metabolism were studied in strains D-402 and D-405 of freshwater colorless sulfur bacteria of the genus Beggiatoa grown organotrophically and mixotrophically .
	manualset3
104308	2	402566	5	NULL	NULL	0	NULL	strains D-402 of freshwater colorless sulfur bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Major pathways of carbon metabolism were studied in strains D-402 and D-405 of freshwater colorless sulfur bacteria of the genus Beggiatoa grown organotrophically and mixotrophically .
	manualset3
104309	3	402566	5	NULL	NULL	0	NULL	strains D-405 of freshwater colorless sulfur bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Major pathways of carbon metabolism were studied in strains D-402 and D-405 of freshwater colorless sulfur bacteria of the genus Beggiatoa grown organotrophically and mixotrophically .
	manualset3
104310	4	402566	5	NULL	NULL	0	NULL	genus Beggiatoa	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Major pathways of carbon metabolism were studied in strains D-402 and D-405 of freshwater colorless sulfur bacteria of the genus Beggiatoa grown organotrophically and mixotrophically .
	manualset3
104311	1	402567	5	NULL	NULL	0	NULL	predictors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Major predictors of LEAD events were diabetes duration , low-density lipoprotein-cholesterol ( LDL-C ) , heart rate , eGDR , log albumin excretion rate ( AER ) , systolic blood pressure ( SBP ) , hypertension , proliferative retinopathy , distal symmetric polyneuropathy , and overt nephropathy ( each P & lt ; .001 ) .
	manualset3
104312	2	402567	5	NULL	NULL	0	NULL	LEAD events	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Major predictors of LEAD events were diabetes duration , low-density lipoprotein-cholesterol ( LDL-C ) , heart rate , eGDR , log albumin excretion rate ( AER ) , systolic blood pressure ( SBP ) , hypertension , proliferative retinopathy , distal symmetric polyneuropathy , and overt nephropathy ( each P & lt ; .001 ) .
	manualset3
104313	3	402567	5	NULL	NULL	NULL	NULL	diabetes duration	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Major predictors of LEAD events were diabetes duration , low-density lipoprotein-cholesterol ( LDL-C ) , heart rate , eGDR , log albumin excretion rate ( AER ) , systolic blood pressure ( SBP ) , hypertension , proliferative retinopathy , distal symmetric polyneuropathy , and overt nephropathy ( each P & lt ; .001 ) .
	manualset3
104314	4	402567	5	NULL	NULL	0	NULL	low-density lipoprotein-cholesterol ( LDL-C )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Major predictors of LEAD events were diabetes duration , low-density lipoprotein-cholesterol ( LDL-C ) , heart rate , eGDR , log albumin excretion rate ( AER ) , systolic blood pressure ( SBP ) , hypertension , proliferative retinopathy , distal symmetric polyneuropathy , and overt nephropathy ( each P & lt ; .001 ) .
	manualset3
104315	5	402567	5	NULL	NULL	0	NULL	heart rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Major predictors of LEAD events were diabetes duration , low-density lipoprotein-cholesterol ( LDL-C ) , heart rate , eGDR , log albumin excretion rate ( AER ) , systolic blood pressure ( SBP ) , hypertension , proliferative retinopathy , distal symmetric polyneuropathy , and overt nephropathy ( each P & lt ; .001 ) .
	manualset3
104316	6	402567	5	NULL	NULL	0	NULL	eGDR	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Major predictors of LEAD events were diabetes duration , low-density lipoprotein-cholesterol ( LDL-C ) , heart rate , eGDR , log albumin excretion rate ( AER ) , systolic blood pressure ( SBP ) , hypertension , proliferative retinopathy , distal symmetric polyneuropathy , and overt nephropathy ( each P & lt ; .001 ) .
	manualset3
104317	7	402567	5	NULL	NULL	0	NULL	log albumin excretion rate ( AER )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Major predictors of LEAD events were diabetes duration , low-density lipoprotein-cholesterol ( LDL-C ) , heart rate , eGDR , log albumin excretion rate ( AER ) , systolic blood pressure ( SBP ) , hypertension , proliferative retinopathy , distal symmetric polyneuropathy , and overt nephropathy ( each P & lt ; .001 ) .
	manualset3
104318	8	402567	5	NULL	NULL	NULL	NULL	systolic blood pressure ( SBP )	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Major predictors of LEAD events were diabetes duration , low-density lipoprotein-cholesterol ( LDL-C ) , heart rate , eGDR , log albumin excretion rate ( AER ) , systolic blood pressure ( SBP ) , hypertension , proliferative retinopathy , distal symmetric polyneuropathy , and overt nephropathy ( each P & lt ; .001 ) .
	manualset3
104319	9	402567	5	NULL	NULL	0	NULL	hypertension 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Major predictors of LEAD events were diabetes duration , low-density lipoprotein-cholesterol ( LDL-C ) , heart rate , eGDR , log albumin excretion rate ( AER ) , systolic blood pressure ( SBP ) , hypertension , proliferative retinopathy , distal symmetric polyneuropathy , and overt nephropathy ( each P & lt ; .001 ) .
	manualset3
104329	10	402567	5	NULL	NULL	0	NULL	proliferative retinopathy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Major predictors of LEAD events were diabetes duration , low-density lipoprotein-cholesterol ( LDL-C ) , heart rate , eGDR , log albumin excretion rate ( AER ) , systolic blood pressure ( SBP ) , hypertension , proliferative retinopathy , distal symmetric polyneuropathy , and overt nephropathy ( each P & lt ; .001 ) .
	manualset3
104330	11	402567	5	NULL	NULL	0	NULL	distal symmetric polyneuropathy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Major predictors of LEAD events were diabetes duration , low-density lipoprotein-cholesterol ( LDL-C ) , heart rate , eGDR , log albumin excretion rate ( AER ) , systolic blood pressure ( SBP ) , hypertension , proliferative retinopathy , distal symmetric polyneuropathy , and overt nephropathy ( each P & lt ; .001 ) .
	manualset3
104331	12	402567	5	NULL	NULL	0	NULL	overt nephropathy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Major predictors of LEAD events were diabetes duration , low-density lipoprotein-cholesterol ( LDL-C ) , heart rate , eGDR , log albumin excretion rate ( AER ) , systolic blood pressure ( SBP ) , hypertension , proliferative retinopathy , distal symmetric polyneuropathy , and overt nephropathy ( each P & lt ; .001 ) .
	manualset3
104332	13	402567	5	NULL	NULL	0	NULL	P & lt ; .001 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Major predictors of LEAD events were diabetes duration , low-density lipoprotein-cholesterol ( LDL-C ) , heart rate , eGDR , log albumin excretion rate ( AER ) , systolic blood pressure ( SBP ) , hypertension , proliferative retinopathy , distal symmetric polyneuropathy , and overt nephropathy ( each P & lt ; .001 ) .
	manualset3
104333	1	402568	5	NULL	NULL	0	NULL	special service costs	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Major special service costs were private duty nursing , medications , medical supplies , respiratory and physical therapy .
	manualset3
104334	2	402568	5	NULL	NULL	0	NULL	 private duty nursing	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Major special service costs were private duty nursing , medications , medical supplies , respiratory and physical therapy .
	manualset3
104339	3	402568	5	NULL	NULL	0	NULL	medications	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Major special service costs were private duty nursing , medications , medical supplies , respiratory and physical therapy .
	manualset3
104340	4	402568	5	NULL	NULL	0	NULL	medical supplies	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Major special service costs were private duty nursing , medications , medical supplies , respiratory and physical therapy .
	manualset3
104341	5	402568	5	NULL	NULL	0	NULL	respiratory therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Major special service costs were private duty nursing , medications , medical supplies , respiratory and physical therapy .
	manualset3
104342	6	402568	5	NULL	NULL	0	NULL	physical therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Major special service costs were private duty nursing , medications , medical supplies , respiratory and physical therapy .
	manualset3
104343	1	402569	5	NULL	NULL	0	NULL	cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Majority of cases ( 58.33 % ) had the development of symptomatic RHD within 2 years of having suffered from RF .
	manualset3
104344	2	402569	5	NULL	NULL	0	NULL	58.33 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Majority of cases ( 58.33 % ) had the development of symptomatic RHD within 2 years of having suffered from RF .
	manualset3
104345	3	402569	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Majority of cases ( 58.33 % ) had the development of symptomatic RHD within 2 years of having suffered from RF .
	manualset3
104347	4	402569	5	NULL	NULL	0	NULL	symptomatic RHD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Majority of cases ( 58.33 % ) had the development of symptomatic RHD within 2 years of having suffered from RF .
	manualset3
104355	5	402569	5	NULL	NULL	0	NULL	2 years	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Majority of cases ( 58.33 % ) had the development of symptomatic RHD within 2 years of having suffered from RF .
	manualset3
104356	6	402569	5	NULL	NULL	0	NULL	RF 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Majority of cases ( 58.33 % ) had the development of symptomatic RHD within 2 years of having suffered from RF .
	manualset3
104357	1	402570	5	NULL	NULL	0	NULL	lemonade 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Making lemonade from lemons : a case study on loss of space at the Dolph Briscoe , Jr. .
	manualset3
104358	2	402570	5	NULL	NULL	NULL	NULL	lemons 	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Making lemonade from lemons : a case study on loss of space at the Dolph Briscoe , Jr. .
	manualset3
104359	3	402570	5	NULL	NULL	0	NULL	case study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Making lemonade from lemons : a case study on loss of space at the Dolph Briscoe , Jr. .
	manualset3
104360	4	402570	5	NULL	NULL	0	NULL	loss of space	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Making lemonade from lemons : a case study on loss of space at the Dolph Briscoe , Jr. .
	manualset3
104361	5	402570	5	NULL	NULL	0	NULL	Dolph Briscoe , Jr.	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Making lemonade from lemons : a case study on loss of space at the Dolph Briscoe , Jr. .
	manualset3
104362	1	402571	5	NULL	NULL	0	NULL	procedures 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Making use of these procedures the authors have been able to maintain a more conservative attitude with regard to the stomach pouch , and to avoid some of the sequellae of the operated stomach .
	manualset3
104363	2	402571	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Making use of these procedures the authors have been able to maintain a more conservative attitude with regard to the stomach pouch , and to avoid some of the sequellae of the operated stomach .
	manualset3
104364	3	402571	5	NULL	NULL	0	NULL	conservative attitude	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Making use of these procedures the authors have been able to maintain a more conservative attitude with regard to the stomach pouch , and to avoid some of the sequellae of the operated stomach .
	manualset3
104365	4	402571	5	NULL	NULL	0	NULL	stomach pouch	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Making use of these procedures the authors have been able to maintain a more conservative attitude with regard to the stomach pouch , and to avoid some of the sequellae of the operated stomach .
	manualset3
104366	5	402571	5	NULL	NULL	0	NULL	sequellae of the operated stomach	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Making use of these procedures the authors have been able to maintain a more conservative attitude with regard to the stomach pouch , and to avoid some of the sequellae of the operated stomach .
	manualset3
104367	1	402572	5	NULL	NULL	0	NULL	Malaria chemoprophylaxis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Malaria chemoprophylaxis and the serologic response to measles and diphtheria-tetanus-whole-cell pertussis vaccines .
	manualset3
104368	2	402572	5	NULL	NULL	0	NULL	serologic response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Malaria chemoprophylaxis and the serologic response to measles and diphtheria-tetanus-whole-cell pertussis vaccines .
	manualset3
104369	3	402572	5	NULL	NULL	NULL	NULL	measles and diphtheria-tetanus-whole-cell pertussis vaccines	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Malaria chemoprophylaxis and the serologic response to measles and diphtheria-tetanus-whole-cell pertussis vaccines .
	manualset3
104370	1	402573	5	NULL	NULL	0	NULL	Malaria control	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Malaria control in a forest fringe area of Assam , India : a pilot study .
	manualset3
104371	2	402573	5	NULL	NULL	0	NULL	forest fringe area	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Malaria control in a forest fringe area of Assam , India : a pilot study .
	manualset3
104372	3	402573	5	NULL	NULL	0	NULL	Assam , India	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Malaria control in a forest fringe area of Assam , India : a pilot study .
	manualset3
104373	4	402573	5	NULL	NULL	0	NULL	pilot study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Malaria control in a forest fringe area of Assam , India : a pilot study .
	manualset3
104374	1	402574	5	NULL	NULL	NULL	NULL	Drosophila homolog of MyD88 ( DmMyD88 )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A Drosophila homolog of MyD88 ( DmMyD88 ) was recently shown to be required for the Toll-mediated immune response .
	manualset3
104375	2	402574	5	NULL	NULL	0	NULL	Toll-mediated immune response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A Drosophila homolog of MyD88 ( DmMyD88 ) was recently shown to be required for the Toll-mediated immune response .
	manualset3
104376	1	402575	5	NULL	NULL	0	NULL	Malaria 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Malaria is a serious and sometimes fatal mosquito-borne disease caused by a protozoan parasite .
	manualset3
104377	2	402575	5	NULL	NULL	0	NULL	mosquito-borne disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Malaria is a serious and sometimes fatal mosquito-borne disease caused by a protozoan parasite .
	manualset3
104378	3	402575	5	NULL	NULL	0	NULL	protozoan parasite	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Malaria is a serious and sometimes fatal mosquito-borne disease caused by a protozoan parasite .
	manualset3
104379	1	402576	5	NULL	NULL	0	NULL	Malaria parasitemia rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Malaria parasitemia rate among schoolchildren ranged from 0-36 .7 % ; the lowest prevalence was observed in the high altitude mountainous range and the highest in the lower altitude plateaux .
	manualset3
104380	2	402576	5	NULL	NULL	0	NULL	schoolchildren 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Malaria parasitemia rate among schoolchildren ranged from 0-36 .7 % ; the lowest prevalence was observed in the high altitude mountainous range and the highest in the lower altitude plateaux .
	manualset3
104382	3	402576	5	NULL	NULL	0	NULL	0-36 .7 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Malaria parasitemia rate among schoolchildren ranged from 0-36 .7 % ; the lowest prevalence was observed in the high altitude mountainous range and the highest in the lower altitude plateaux .
	manualset3
104383	4	402576	5	NULL	NULL	0	NULL	lowest prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Malaria parasitemia rate among schoolchildren ranged from 0-36 .7 % ; the lowest prevalence was observed in the high altitude mountainous range and the highest in the lower altitude plateaux .
	manualset3
104384	5	402576	5	NULL	NULL	0	NULL	high altitude mountainous range	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Malaria parasitemia rate among schoolchildren ranged from 0-36 .7 % ; the lowest prevalence was observed in the high altitude mountainous range and the highest in the lower altitude plateaux .
	manualset3
104385	6	402576	5	NULL	NULL	0	NULL	lower altitude plateaux	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Malaria parasitemia rate among schoolchildren ranged from 0-36 .7 % ; the lowest prevalence was observed in the high altitude mountainous range and the highest in the lower altitude plateaux .
	manualset3
104390	1	402577	5	NULL	NULL	0	NULL	Male-induced oestrus	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Male-induced oestrus and ovulation in female brush-tailed bettongs ( Bettongia penicillata ) suckling a young in the pouch .
	manualset3
104392	2	402577	5	NULL	NULL	0	NULL	Male-induced ovulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Male-induced oestrus and ovulation in female brush-tailed bettongs ( Bettongia penicillata ) suckling a young in the pouch .
	manualset3
104394	3	402577	5	NULL	NULL	0	NULL	female brush-tailed bettongs (Bettongia penicillata)	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Male-induced oestrus and ovulation in female brush-tailed bettongs ( Bettongia penicillata ) suckling a young in the pouch .
	manualset3
104395	4	402577	5	NULL	NULL	0	NULL	suckling 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Male-induced oestrus and ovulation in female brush-tailed bettongs ( Bettongia penicillata ) suckling a young in the pouch .
	manualset3
104396	5	402577	5	NULL	NULL	0	NULL	young 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Male-induced oestrus and ovulation in female brush-tailed bettongs ( Bettongia penicillata ) suckling a young in the pouch .
	manualset3
104397	6	402577	5	NULL	NULL	0	NULL	pouch 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Male-induced oestrus and ovulation in female brush-tailed bettongs ( Bettongia penicillata ) suckling a young in the pouch .
	manualset3
104401	1	402578	5	NULL	NULL	0	NULL	Male SD ( Crj : CD )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Male SD ( Crj : CD ) , Lewis ( LEW/Crj ) , WKY ( WKY/NCrj ) , Wistar ( Crj : Wistar ) and F344 ( F344/DuCrj ) animals were given drinking water containing 100 micrograms/ml of MNNG for 30 weeks and were killed at week 50 .
	manualset3
104402	2	402578	5	NULL	NULL	0	NULL	 Lewis ( LEW/Crj )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Male SD ( Crj : CD ) , Lewis ( LEW/Crj ) , WKY ( WKY/NCrj ) , Wistar ( Crj : Wistar ) and F344 ( F344/DuCrj ) animals were given drinking water containing 100 micrograms/ml of MNNG for 30 weeks and were killed at week 50 .
	manualset3
104403	3	402578	5	NULL	NULL	0	NULL	WKY ( WKY/NCrj )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Male SD ( Crj : CD ) , Lewis ( LEW/Crj ) , WKY ( WKY/NCrj ) , Wistar ( Crj : Wistar ) and F344 ( F344/DuCrj ) animals were given drinking water containing 100 micrograms/ml of MNNG for 30 weeks and were killed at week 50 .
	manualset3
104404	4	402578	5	NULL	NULL	0	NULL	Wistar ( Crj : Wistar ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Male SD ( Crj : CD ) , Lewis ( LEW/Crj ) , WKY ( WKY/NCrj ) , Wistar ( Crj : Wistar ) and F344 ( F344/DuCrj ) animals were given drinking water containing 100 micrograms/ml of MNNG for 30 weeks and were killed at week 50 .
	manualset3
104405	5	402578	5	NULL	NULL	0	NULL	F344 ( F344/DuCrj ) animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Male SD ( Crj : CD ) , Lewis ( LEW/Crj ) , WKY ( WKY/NCrj ) , Wistar ( Crj : Wistar ) and F344 ( F344/DuCrj ) animals were given drinking water containing 100 micrograms/ml of MNNG for 30 weeks and were killed at week 50 .
	manualset3
104406	6	402578	5	NULL	NULL	0	NULL	drinking water	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Male SD ( Crj : CD ) , Lewis ( LEW/Crj ) , WKY ( WKY/NCrj ) , Wistar ( Crj : Wistar ) and F344 ( F344/DuCrj ) animals were given drinking water containing 100 micrograms/ml of MNNG for 30 weeks and were killed at week 50 .
	manualset3
104407	7	402578	5	NULL	NULL	0	NULL	100 micrograms/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Male SD ( Crj : CD ) , Lewis ( LEW/Crj ) , WKY ( WKY/NCrj ) , Wistar ( Crj : Wistar ) and F344 ( F344/DuCrj ) animals were given drinking water containing 100 micrograms/ml of MNNG for 30 weeks and were killed at week 50 .
	manualset3
104408	8	402578	5	NULL	NULL	0	NULL	MNNG 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Male SD ( Crj : CD ) , Lewis ( LEW/Crj ) , WKY ( WKY/NCrj ) , Wistar ( Crj : Wistar ) and F344 ( F344/DuCrj ) animals were given drinking water containing 100 micrograms/ml of MNNG for 30 weeks and were killed at week 50 .
	manualset3
104409	9	402578	5	NULL	NULL	0	NULL	30 weeks	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Male SD ( Crj : CD ) , Lewis ( LEW/Crj ) , WKY ( WKY/NCrj ) , Wistar ( Crj : Wistar ) and F344 ( F344/DuCrj ) animals were given drinking water containing 100 micrograms/ml of MNNG for 30 weeks and were killed at week 50 .
	manualset3
104410	10	402578	5	NULL	NULL	0	NULL	week 50	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Male SD ( Crj : CD ) , Lewis ( LEW/Crj ) , WKY ( WKY/NCrj ) , Wistar ( Crj : Wistar ) and F344 ( F344/DuCrj ) animals were given drinking water containing 100 micrograms/ml of MNNG for 30 weeks and were killed at week 50 .
	manualset3
104411	1	402579	5	NULL	NULL	0	NULL	Male Sprague-Dawley rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Male Sprague-Dawley rats were fed an AIN-93G diet containing soybean oil for 4 wk .
	manualset3
104412	2	402579	5	NULL	NULL	0	NULL	AIN-93G diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Male Sprague-Dawley rats were fed an AIN-93G diet containing soybean oil for 4 wk .
	manualset3
104413	3	402579	5	NULL	NULL	0	NULL	soybean oil	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Male Sprague-Dawley rats were fed an AIN-93G diet containing soybean oil for 4 wk .
	manualset3
104414	4	402579	5	NULL	NULL	0	NULL	4 wk	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Male Sprague-Dawley rats were fed an AIN-93G diet containing soybean oil for 4 wk .
	manualset3
104415	1	402580	5	NULL	NULL	0	NULL	Male Sprague-Dawley rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Male Sprague-Dawley rats were used to measure the brain uptake index ( BUI ) by single-pass clearance in brain after rapid injection at pH 7.4 into the left common carotid artery ( expressed as a percentage ) relative to simultaneously injected 3HOH .
	manualset3
104416	2	402580	5	NULL	NULL	NULL	NULL	brain uptake index ( BUI )	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Male Sprague-Dawley rats were used to measure the brain uptake index ( BUI ) by single-pass clearance in brain after rapid injection at pH 7.4 into the left common carotid artery ( expressed as a percentage ) relative to simultaneously injected 3HOH .
	manualset3
104418	3	402580	5	NULL	NULL	0	NULL	single-pass clearance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Male Sprague-Dawley rats were used to measure the brain uptake index ( BUI ) by single-pass clearance in brain after rapid injection at pH 7.4 into the left common carotid artery ( expressed as a percentage ) relative to simultaneously injected 3HOH .
	manualset3
104419	4	402580	5	NULL	NULL	0	NULL	brain 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Male Sprague-Dawley rats were used to measure the brain uptake index ( BUI ) by single-pass clearance in brain after rapid injection at pH 7.4 into the left common carotid artery ( expressed as a percentage ) relative to simultaneously injected 3HOH .
	manualset3
104420	5	402580	5	NULL	NULL	0	NULL	rapid injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Male Sprague-Dawley rats were used to measure the brain uptake index ( BUI ) by single-pass clearance in brain after rapid injection at pH 7.4 into the left common carotid artery ( expressed as a percentage ) relative to simultaneously injected 3HOH .
	manualset3
104421	6	402580	5	NULL	NULL	0	NULL	pH 7.4	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Male Sprague-Dawley rats were used to measure the brain uptake index ( BUI ) by single-pass clearance in brain after rapid injection at pH 7.4 into the left common carotid artery ( expressed as a percentage ) relative to simultaneously injected 3HOH .
	manualset3
104423	7	402580	5	NULL	NULL	0	NULL	left common carotid artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Male Sprague-Dawley rats were used to measure the brain uptake index ( BUI ) by single-pass clearance in brain after rapid injection at pH 7.4 into the left common carotid artery ( expressed as a percentage ) relative to simultaneously injected 3HOH .
	manualset3
104424	8	402580	5	NULL	NULL	0	NULL	percentage 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Male Sprague-Dawley rats were used to measure the brain uptake index ( BUI ) by single-pass clearance in brain after rapid injection at pH 7.4 into the left common carotid artery ( expressed as a percentage ) relative to simultaneously injected 3HOH .
	manualset3
104426	9	402580	5	NULL	NULL	0	NULL	3HOH 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Male Sprague-Dawley rats were used to measure the brain uptake index ( BUI ) by single-pass clearance in brain after rapid injection at pH 7.4 into the left common carotid artery ( expressed as a percentage ) relative to simultaneously injected 3HOH .
	manualset3
104427	1	402581	5	NULL	NULL	0	NULL	Male blood donors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Male blood donors from three population groups ( Indian , Black , White ) who showed neither microcytosis nor levels of serum ferritin or transferrin saturation suggestive of iron deficiency were matched in 3 's 1 from each population , for age , number of previous blood donations , and serum ferritin .
	manualset3
104428	2	402581	5	NULL	NULL	0	NULL	population groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Male blood donors from three population groups ( Indian , Black , White ) who showed neither microcytosis nor levels of serum ferritin or transferrin saturation suggestive of iron deficiency were matched in 3 's 1 from each population , for age , number of previous blood donations , and serum ferritin .
	manualset3
104429	3	402581	5	NULL	NULL	0	NULL	Indian 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Male blood donors from three population groups ( Indian , Black , White ) who showed neither microcytosis nor levels of serum ferritin or transferrin saturation suggestive of iron deficiency were matched in 3 's 1 from each population , for age , number of previous blood donations , and serum ferritin .
	manualset3
104430	4	402581	5	NULL	NULL	0	NULL	Black 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Male blood donors from three population groups ( Indian , Black , White ) who showed neither microcytosis nor levels of serum ferritin or transferrin saturation suggestive of iron deficiency were matched in 3 's 1 from each population , for age , number of previous blood donations , and serum ferritin .
	manualset3
104431	5	402581	5	NULL	NULL	0	NULL	White 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Male blood donors from three population groups ( Indian , Black , White ) who showed neither microcytosis nor levels of serum ferritin or transferrin saturation suggestive of iron deficiency were matched in 3 's 1 from each population , for age , number of previous blood donations , and serum ferritin .
	manualset3
104432	6	402581	5	NULL	NULL	0	NULL	microcytosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Male blood donors from three population groups ( Indian , Black , White ) who showed neither microcytosis nor levels of serum ferritin or transferrin saturation suggestive of iron deficiency were matched in 3 's 1 from each population , for age , number of previous blood donations , and serum ferritin .
	manualset3
104433	7	402581	5	NULL	NULL	0	NULL	levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Male blood donors from three population groups ( Indian , Black , White ) who showed neither microcytosis nor levels of serum ferritin or transferrin saturation suggestive of iron deficiency were matched in 3 's 1 from each population , for age , number of previous blood donations , and serum ferritin .
	manualset3
104438	8	402581	5	NULL	NULL	0	NULL	serum ferritin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Male blood donors from three population groups ( Indian , Black , White ) who showed neither microcytosis nor levels of serum ferritin or transferrin saturation suggestive of iron deficiency were matched in 3 's 1 from each population , for age , number of previous blood donations , and serum ferritin .
	manualset3
104439	9	402581	5	NULL	NULL	0	NULL	transferrin saturation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Male blood donors from three population groups ( Indian , Black , White ) who showed neither microcytosis nor levels of serum ferritin or transferrin saturation suggestive of iron deficiency were matched in 3 's 1 from each population , for age , number of previous blood donations , and serum ferritin .
	manualset3
104440	10	402581	5	NULL	NULL	0	NULL	iron deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Male blood donors from three population groups ( Indian , Black , White ) who showed neither microcytosis nor levels of serum ferritin or transferrin saturation suggestive of iron deficiency were matched in 3 's 1 from each population , for age , number of previous blood donations , and serum ferritin .
	manualset3
104441	11	402581	5	NULL	NULL	0	NULL	3 's 1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Male blood donors from three population groups ( Indian , Black , White ) who showed neither microcytosis nor levels of serum ferritin or transferrin saturation suggestive of iron deficiency were matched in 3 's 1 from each population , for age , number of previous blood donations , and serum ferritin .
	manualset3
104442	12	402581	5	NULL	NULL	0	NULL	population 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Male blood donors from three population groups ( Indian , Black , White ) who showed neither microcytosis nor levels of serum ferritin or transferrin saturation suggestive of iron deficiency were matched in 3 's 1 from each population , for age , number of previous blood donations , and serum ferritin .
	manualset3
104443	13	402581	5	NULL	NULL	0	NULL	age 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Male blood donors from three population groups ( Indian , Black , White ) who showed neither microcytosis nor levels of serum ferritin or transferrin saturation suggestive of iron deficiency were matched in 3 's 1 from each population , for age , number of previous blood donations , and serum ferritin .
	manualset3
104444	14	402581	5	NULL	NULL	0	NULL	number of previous blood donations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Male blood donors from three population groups ( Indian , Black , White ) who showed neither microcytosis nor levels of serum ferritin or transferrin saturation suggestive of iron deficiency were matched in 3 's 1 from each population , for age , number of previous blood donations , and serum ferritin .
	manualset3
104445	15	402581	5	NULL	NULL	0	NULL	serum ferritin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Male blood donors from three population groups ( Indian , Black , White ) who showed neither microcytosis nor levels of serum ferritin or transferrin saturation suggestive of iron deficiency were matched in 3 's 1 from each population , for age , number of previous blood donations , and serum ferritin .
	manualset3
104451	1	402582	5	NULL	NULL	0	NULL	Male Wistar rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Male Wistar rats ( 250-280 g ) were injected with DMTI-II ( 1-100microg / cavity ) , and at 4-24h thereafter the leukocyte counts in peritoneal lavage were evaluated .
	manualset3
104460	2	402582	5	NULL	NULL	0	NULL	250-280 g	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Male Wistar rats ( 250-280 g ) were injected with DMTI-II ( 1-100microg / cavity ) , and at 4-24h thereafter the leukocyte counts in peritoneal lavage were evaluated .
	manualset3
104463	3	402582	5	NULL	NULL	0	NULL	DMTI-II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Male Wistar rats ( 250-280 g ) were injected with DMTI-II ( 1-100microg / cavity ) , and at 4-24h thereafter the leukocyte counts in peritoneal lavage were evaluated .
	manualset3
104464	4	402582	5	NULL	NULL	0	NULL	1-100microg / cavity 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Male Wistar rats ( 250-280 g ) were injected with DMTI-II ( 1-100microg / cavity ) , and at 4-24h thereafter the leukocyte counts in peritoneal lavage were evaluated .
	manualset3
104466	5	402582	5	NULL	NULL	0	NULL	4-24h 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Male Wistar rats ( 250-280 g ) were injected with DMTI-II ( 1-100microg / cavity ) , and at 4-24h thereafter the leukocyte counts in peritoneal lavage were evaluated .
	manualset3
104468	6	402582	5	NULL	NULL	0	NULL	leukocyte counts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Male Wistar rats ( 250-280 g ) were injected with DMTI-II ( 1-100microg / cavity ) , and at 4-24h thereafter the leukocyte counts in peritoneal lavage were evaluated .
	manualset3
104473	7	402582	5	NULL	NULL	0	NULL	peritoneal lavage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Male Wistar rats ( 250-280 g ) were injected with DMTI-II ( 1-100microg / cavity ) , and at 4-24h thereafter the leukocyte counts in peritoneal lavage were evaluated .
	manualset3
104475	1	402583	5	NULL	NULL	0	NULL	Male Wistar rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Male Wistar rats were treated with water , cyclophosphamide ( CP ) 40 mg/kg , and ribavirin 20 , 100 and 200 mg/kg ( i.p. ) for 5 consecutive days at intervals of 24h .
	manualset3
104476	2	402583	5	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Male Wistar rats were treated with water , cyclophosphamide ( CP ) 40 mg/kg , and ribavirin 20 , 100 and 200 mg/kg ( i.p. ) for 5 consecutive days at intervals of 24h .
	manualset3
104477	3	402583	5	NULL	NULL	0	NULL	cyclophosphamide ( CP ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Male Wistar rats were treated with water , cyclophosphamide ( CP ) 40 mg/kg , and ribavirin 20 , 100 and 200 mg/kg ( i.p. ) for 5 consecutive days at intervals of 24h .
	manualset3
104478	4	402583	5	NULL	NULL	0	NULL	40 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Male Wistar rats were treated with water , cyclophosphamide ( CP ) 40 mg/kg , and ribavirin 20 , 100 and 200 mg/kg ( i.p. ) for 5 consecutive days at intervals of 24h .
	manualset3
104479	5	402583	5	NULL	NULL	0	NULL	ribavirin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Male Wistar rats were treated with water , cyclophosphamide ( CP ) 40 mg/kg , and ribavirin 20 , 100 and 200 mg/kg ( i.p. ) for 5 consecutive days at intervals of 24h .
	manualset3
104480	6	402583	5	NULL	NULL	0	NULL	20 , 100 and 200 mg/kg ( i.p. )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Male Wistar rats were treated with water , cyclophosphamide ( CP ) 40 mg/kg , and ribavirin 20 , 100 and 200 mg/kg ( i.p. ) for 5 consecutive days at intervals of 24h .
	manualset3
104481	7	402583	5	NULL	NULL	0	NULL	5 consecutive days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Male Wistar rats were treated with water , cyclophosphamide ( CP ) 40 mg/kg , and ribavirin 20 , 100 and 200 mg/kg ( i.p. ) for 5 consecutive days at intervals of 24h .
	manualset3
104482	8	402583	5	NULL	NULL	0	NULL	intervals 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Male Wistar rats were treated with water , cyclophosphamide ( CP ) 40 mg/kg , and ribavirin 20 , 100 and 200 mg/kg ( i.p. ) for 5 consecutive days at intervals of 24h .
	manualset3
104483	9	402583	5	NULL	NULL	0	NULL	24h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Male Wistar rats were treated with water , cyclophosphamide ( CP ) 40 mg/kg , and ribavirin 20 , 100 and 200 mg/kg ( i.p. ) for 5 consecutive days at intervals of 24h .
	manualset3
104484	1	402584	5	NULL	NULL	0	NULL	GPI-anchored protein deficient population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A GPI-anchored protein deficient population was identified in 15 % ( 17/111 ) of patients with AA who had a negative Ham 's test and no laboratory evidence of hemolysis .
	manualset3
104485	2	402584	5	NULL	NULL	0	NULL	15 % ( 17/111 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A GPI-anchored protein deficient population was identified in 15 % ( 17/111 ) of patients with AA who had a negative Ham 's test and no laboratory evidence of hemolysis .
	manualset3
104486	3	402584	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A GPI-anchored protein deficient population was identified in 15 % ( 17/111 ) of patients with AA who had a negative Ham 's test and no laboratory evidence of hemolysis .
	manualset3
104487	4	402584	5	NULL	NULL	0	NULL	AA	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A GPI-anchored protein deficient population was identified in 15 % ( 17/111 ) of patients with AA who had a negative Ham 's test and no laboratory evidence of hemolysis .
	manualset3
104488	5	402584	5	NULL	NULL	NULL	NULL	negative Ham 's test	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A GPI-anchored protein deficient population was identified in 15 % ( 17/111 ) of patients with AA who had a negative Ham 's test and no laboratory evidence of hemolysis .
	manualset3
104489	6	402584	5	NULL	NULL	0	NULL	laboratory evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A GPI-anchored protein deficient population was identified in 15 % ( 17/111 ) of patients with AA who had a negative Ham 's test and no laboratory evidence of hemolysis .
	manualset3
104490	7	402584	5	NULL	NULL	0	NULL	hemolysis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A GPI-anchored protein deficient population was identified in 15 % ( 17/111 ) of patients with AA who had a negative Ham 's test and no laboratory evidence of hemolysis .
	manualset3
104491	1	402585	5	NULL	NULL	0	NULL	Males 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Males , but not females , exhibited a circadian variation in metabolite levels .
	manualset3
104492	2	402585	5	NULL	NULL	0	NULL	females 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Males , but not females , exhibited a circadian variation in metabolite levels .
	manualset3
104493	3	402585	5	NULL	NULL	0	NULL	circadian variation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Males , but not females , exhibited a circadian variation in metabolite levels .
	manualset3
104494	4	402585	5	NULL	NULL	0	NULL	metabolite levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Males , but not females , exhibited a circadian variation in metabolite levels .
	manualset3
104495	1	402586	5	NULL	NULL	0	NULL	Malignant-appearing lesions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Malignant-appearing lesions usually require biopsy by the least invasive route appropriate for the suspected tumor type .
	manualset3
104496	2	402586	5	NULL	NULL	0	NULL	biopsy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Malignant-appearing lesions usually require biopsy by the least invasive route appropriate for the suspected tumor type .
	manualset3
104497	3	402586	5	NULL	NULL	0	NULL	least invasive route appropriate	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Malignant-appearing lesions usually require biopsy by the least invasive route appropriate for the suspected tumor type .
	manualset3
104498	4	402586	5	NULL	NULL	0	NULL	suspected tumor type	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Malignant-appearing lesions usually require biopsy by the least invasive route appropriate for the suspected tumor type .
	manualset3
104499	1	402587	5	NULL	NULL	0	NULL	Malignant huaman breast tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Malignant and benign human breast tumors as well as rabbit breast tissue were examined for specific receptors for 1 , 25-dihydroxyvitamin D3 using competitive binding studies and sucrose density gradient analysis .
	manualset3
104500	2	402587	5	NULL	NULL	0	NULL	benign human breast tumors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Malignant and benign human breast tumors as well as rabbit breast tissue were examined for specific receptors for 1 , 25-dihydroxyvitamin D3 using competitive binding studies and sucrose density gradient analysis .
	manualset3
104501	3	402587	5	NULL	NULL	0	NULL	rabbit breast tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Malignant and benign human breast tumors as well as rabbit breast tissue were examined for specific receptors for 1 , 25-dihydroxyvitamin D3 using competitive binding studies and sucrose density gradient analysis .
	manualset3
104502	4	402587	5	NULL	NULL	0	NULL	specific receptors 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Malignant and benign human breast tumors as well as rabbit breast tissue were examined for specific receptors for 1 , 25-dihydroxyvitamin D3 using competitive binding studies and sucrose density gradient analysis .
	manualset3
104503	5	402587	5	NULL	NULL	0	NULL	1 , 25-dihydroxyvitamin D3	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Malignant and benign human breast tumors as well as rabbit breast tissue were examined for specific receptors for 1 , 25-dihydroxyvitamin D3 using competitive binding studies and sucrose density gradient analysis .
	manualset3
104504	6	402587	5	NULL	NULL	0	NULL	competitive binding studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Malignant and benign human breast tumors as well as rabbit breast tissue were examined for specific receptors for 1 , 25-dihydroxyvitamin D3 using competitive binding studies and sucrose density gradient analysis .
	manualset3
104505	7	402587	5	NULL	NULL	0	NULL	sucrose density gradient analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Malignant and benign human breast tumors as well as rabbit breast tissue were examined for specific receptors for 1 , 25-dihydroxyvitamin D3 using competitive binding studies and sucrose density gradient analysis .
	manualset3
104506	1	402588	5	NULL	NULL	0	NULL	Malignant cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Malignant cells require iron , and exhibit more transferrin receptors .
	manualset3
104507	2	402588	5	NULL	NULL	0	NULL	iron 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Malignant cells require iron , and exhibit more transferrin receptors .
	manualset3
104508	3	402588	5	NULL	NULL	0	NULL	transferrin receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Malignant cells require iron , and exhibit more transferrin receptors .
	manualset3
104509	1	402589	5	NULL	NULL	0	NULL	Malignant fibrous histiocytoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Malignant fibrous histiocytoma of bone following primitive neuroectodermal tumor of bone .
	manualset3
104510	2	402589	5	NULL	NULL	0	NULL	bone 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Malignant fibrous histiocytoma of bone following primitive neuroectodermal tumor of bone .
	manualset3
104511	3	402589	5	NULL	NULL	0	NULL	primitive neuroectodermal tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Malignant fibrous histiocytoma of bone following primitive neuroectodermal tumor of bone .
	manualset3
104512	4	402589	5	NULL	NULL	0	NULL	bone	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Malignant fibrous histiocytoma of bone following primitive neuroectodermal tumor of bone .
	manualset3
104513	1	402590	5	NULL	NULL	0	NULL	Malignant gliomas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Malignant gliomas are characterized by its invasiveness and dissemination , resulting in frequent tumor recurrence after surgical resection and/or conventional chemotherapy and radiation therapy .
	manualset3
104514	2	402590	5	NULL	NULL	NULL	NULL	invasiveness 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Malignant gliomas are characterized by its invasiveness and dissemination , resulting in frequent tumor recurrence after surgical resection and/or conventional chemotherapy and radiation therapy .
	manualset3
104515	3	402590	5	NULL	NULL	0	NULL	dissemination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Malignant gliomas are characterized by its invasiveness and dissemination , resulting in frequent tumor recurrence after surgical resection and/or conventional chemotherapy and radiation therapy .
	manualset3
104516	4	402590	5	NULL	NULL	0	NULL	frequent tumor recurrence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Malignant gliomas are characterized by its invasiveness and dissemination , resulting in frequent tumor recurrence after surgical resection and/or conventional chemotherapy and radiation therapy .
	manualset3
104517	5	402590	5	NULL	NULL	0	NULL	surgical resection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Malignant gliomas are characterized by its invasiveness and dissemination , resulting in frequent tumor recurrence after surgical resection and/or conventional chemotherapy and radiation therapy .
	manualset3
104518	6	402590	5	NULL	NULL	0	NULL	conventional chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Malignant gliomas are characterized by its invasiveness and dissemination , resulting in frequent tumor recurrence after surgical resection and/or conventional chemotherapy and radiation therapy .
	manualset3
104519	7	402590	5	NULL	NULL	0	NULL	radiation therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Malignant gliomas are characterized by its invasiveness and dissemination , resulting in frequent tumor recurrence after surgical resection and/or conventional chemotherapy and radiation therapy .
	manualset3
104520	1	402591	5	NULL	NULL	NULL	NULL	Malignant pheochromocytoma	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Malignant pheochromocytoma treated by I-131 MIBG .
	manualset3
104521	2	402591	5	NULL	NULL	NULL	NULL	I-131 MIBG 	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Malignant pheochromocytoma treated by I-131 MIBG .
	manualset3
104522	1	402592	5	NULL	NULL	0	NULL	Malignant seminoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Malignant seminoma in a cryptorchid stallion .
	manualset3
104523	2	402592	5	NULL	NULL	0	NULL	cryptorchid stallion	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Malignant seminoma in a cryptorchid stallion .
	manualset3
104524	1	402593	5	NULL	NULL	0	NULL	Malnutrition 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Malnutrition associated with critical illness has been unequivocally associated with increased morbidity and mortality in humans .
	manualset3
104525	2	402593	5	NULL	NULL	0	NULL	critical illness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Malnutrition associated with critical illness has been unequivocally associated with increased morbidity and mortality in humans .
	manualset3
104526	3	402593	5	NULL	NULL	0	NULL	increased morbidity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Malnutrition associated with critical illness has been unequivocally associated with increased morbidity and mortality in humans .
	manualset3
104527	4	402593	5	NULL	NULL	0	NULL	mortality 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Malnutrition associated with critical illness has been unequivocally associated with increased morbidity and mortality in humans .
	manualset3
104528	5	402593	5	NULL	NULL	NULL	NULL	humans 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Malnutrition associated with critical illness has been unequivocally associated with increased morbidity and mortality in humans .
	manualset3
104529	1	402594	5	NULL	NULL	0	NULL	Malnutrition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Malnutrition in this population , as reflected by anemia , appears primarily attributable to food shortages and inadequate traditional feeding practices .
	manualset3
104530	2	402594	5	NULL	NULL	0	NULL	population 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Malnutrition in this population , as reflected by anemia , appears primarily attributable to food shortages and inadequate traditional feeding practices .
	manualset3
104531	3	402594	5	NULL	NULL	0	NULL	anemia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Malnutrition in this population , as reflected by anemia , appears primarily attributable to food shortages and inadequate traditional feeding practices .
	manualset3
104532	4	402594	5	NULL	NULL	0	NULL	food shortages	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Malnutrition in this population , as reflected by anemia , appears primarily attributable to food shortages and inadequate traditional feeding practices .
	manualset3
104533	5	402594	5	NULL	NULL	0	NULL	inadequate traditional feeding practices	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Malnutrition in this population , as reflected by anemia , appears primarily attributable to food shortages and inadequate traditional feeding practices .
	manualset3
104534	1	402595	5	NULL	NULL	0	NULL	Malonaldehyde formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Malonaldehyde formation and DNA fragmentation : two independent sperm decays linked to reactive oxygen species .
	manualset3
104535	2	402595	5	NULL	NULL	0	NULL	DNA fragmentation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Malonaldehyde formation and DNA fragmentation : two independent sperm decays linked to reactive oxygen species .
	manualset3
104536	3	402595	5	NULL	NULL	0	NULL	two independent sperm decays	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Malonaldehyde formation and DNA fragmentation : two independent sperm decays linked to reactive oxygen species .
	manualset3
104537	4	402595	5	NULL	NULL	0	NULL	reactive oxygen species	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Malonaldehyde formation and DNA fragmentation : two independent sperm decays linked to reactive oxygen species .
	manualset3
104538	1	402596	5	NULL	NULL	0	NULL	Malunions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Malunions of the distal radius : treatment options .
	manualset3
104539	2	402596	5	NULL	NULL	0	NULL	distal radius 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Malunions of the distal radius : treatment options .
	manualset3
104540	3	402596	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Malunions of the distal radius : treatment options .
	manualset3
104541	1	402597	5	NULL	NULL	0	NULL	Mammary gland expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mammary gland expression of antibacterial peptide genes to inhibit bacterial pathogens causing mastitis .
	manualset3
104542	2	402597	5	NULL	NULL	0	NULL	antibacterial peptide genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mammary gland expression of antibacterial peptide genes to inhibit bacterial pathogens causing mastitis .
	manualset3
104543	3	402597	5	NULL	NULL	0	NULL	bacterial pathogens 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mammary gland expression of antibacterial peptide genes to inhibit bacterial pathogens causing mastitis .
	manualset3
104544	4	402597	5	NULL	NULL	NULL	NULL	mastitis 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mammary gland expression of antibacterial peptide genes to inhibit bacterial pathogens causing mastitis .
	manualset3
104545	1	402598	5	NULL	NULL	0	NULL	Management 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Management of Mirizzi syndrome by laparoscopic cholecystectomy and laparoscopic ultrasonography .
	manualset3
104546	2	402598	5	NULL	NULL	0	NULL	Mirizzi syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Management of Mirizzi syndrome by laparoscopic cholecystectomy and laparoscopic ultrasonography .
	manualset3
104547	3	402598	5	NULL	NULL	0	NULL	laparoscopic cholecystectomy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Management of Mirizzi syndrome by laparoscopic cholecystectomy and laparoscopic ultrasonography .
	manualset3
104548	4	402598	5	NULL	NULL	0	NULL	laparoscopic ultrasonography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Management of Mirizzi syndrome by laparoscopic cholecystectomy and laparoscopic ultrasonography .
	manualset3
104549	1	402599	5	NULL	NULL	0	NULL	Management 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Management should be directed toward investigation and correction of deranged physiology and appropriate monitoring of maternal-feto-placental status .
	manualset3
104550	2	402599	5	NULL	NULL	0	NULL	investigation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Management should be directed toward investigation and correction of deranged physiology and appropriate monitoring of maternal-feto-placental status .
	manualset3
104551	3	402599	5	NULL	NULL	0	NULL	correction 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Management should be directed toward investigation and correction of deranged physiology and appropriate monitoring of maternal-feto-placental status .
	manualset3
104552	4	402599	5	NULL	NULL	0	NULL	deranged physiology 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Management should be directed toward investigation and correction of deranged physiology and appropriate monitoring of maternal-feto-placental status .
	manualset3
104553	6	402599	5	NULL	NULL	NULL	NULL	maternal-feto-placental status	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Management should be directed toward investigation and correction of deranged physiology and appropriate monitoring of maternal-feto-placental status .
	manualset3
112971	5	402599	5	NULL	NULL	0	NULL	monitoring 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Management should be directed toward investigation and correction of deranged physiology and appropriate monitoring of maternal-feto-placental status .
	manualset3
104554	1	402600	5	NULL	NULL	0	NULL	Management 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Management consists of making the patient and relatives aware about the causation and diagnosis .
	manualset3
104555	2	402600	5	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Management consists of making the patient and relatives aware about the causation and diagnosis .
	manualset3
104556	3	402600	5	NULL	NULL	0	NULL	relatives 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Management consists of making the patient and relatives aware about the causation and diagnosis .
	manualset3
104557	4	402600	5	NULL	NULL	0	NULL	causation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Management consists of making the patient and relatives aware about the causation and diagnosis .
	manualset3
104558	5	402600	5	NULL	NULL	NULL	NULL	diagnosis 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Management consists of making the patient and relatives aware about the causation and diagnosis .
	manualset3
104559	1	402601	5	NULL	NULL	0	NULL	Management evaluation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Management evaluation must be specific , comprehensive , and targeted by scientific studies , risk group and temporal analyses , physical examination , and laboratory diagnosis .
	manualset3
104560	2	402601	5	NULL	NULL	0	NULL	scientific studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Management evaluation must be specific , comprehensive , and targeted by scientific studies , risk group and temporal analyses , physical examination , and laboratory diagnosis .
	manualset3
104561	3	402601	5	NULL	NULL	0	NULL	risk group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Management evaluation must be specific , comprehensive , and targeted by scientific studies , risk group and temporal analyses , physical examination , and laboratory diagnosis .
	manualset3
104562	4	402601	5	NULL	NULL	0	NULL	temporal analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Management evaluation must be specific , comprehensive , and targeted by scientific studies , risk group and temporal analyses , physical examination , and laboratory diagnosis .
	manualset3
104563	5	402601	5	NULL	NULL	0	NULL	physical examination 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Management evaluation must be specific , comprehensive , and targeted by scientific studies , risk group and temporal analyses , physical examination , and laboratory diagnosis .
	manualset3
104564	6	402601	5	NULL	NULL	NULL	NULL	laboratory diagnosis	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Management evaluation must be specific , comprehensive , and targeted by scientific studies , risk group and temporal analyses , physical examination , and laboratory diagnosis .
	manualset3
104565	1	402602	5	NULL	NULL	0	NULL	Management 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Management of intravaginal warts in women with 5-fluorouracil ( 1 % ) in vaginal hydrophilic gel : a placebo-controlled double-blind study .
	manualset3
104566	2	402602	5	NULL	NULL	0	NULL	intravaginal warts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Management of intravaginal warts in women with 5-fluorouracil ( 1 % ) in vaginal hydrophilic gel : a placebo-controlled double-blind study .
	manualset3
104567	3	402602	5	NULL	NULL	0	NULL	women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Management of intravaginal warts in women with 5-fluorouracil ( 1 % ) in vaginal hydrophilic gel : a placebo-controlled double-blind study .
	manualset3
104568	4	402602	5	NULL	NULL	NULL	NULL	5-fluorouracil in vaginal hydrophilic gel 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Management of intravaginal warts in women with 5-fluorouracil ( 1 % ) in vaginal hydrophilic gel : a placebo-controlled double-blind study .
	manualset3
104569	5	402602	5	NULL	NULL	0	NULL	1%	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Management of intravaginal warts in women with 5-fluorouracil ( 1 % ) in vaginal hydrophilic gel : a placebo-controlled double-blind study .
	manualset3
104570	6	402602	5	NULL	NULL	0	NULL	placebo-controlled double-blind study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Management of intravaginal warts in women with 5-fluorouracil ( 1 % ) in vaginal hydrophilic gel : a placebo-controlled double-blind study .
	manualset3
104571	1	402603	5	NULL	NULL	0	NULL	Management 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Management of postoperative peritonitis after anterior resection : experience from a referral intensive care unit .
	manualset3
104572	2	402603	5	NULL	NULL	NULL	NULL	postoperative peritonitis 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Management of postoperative peritonitis after anterior resection : experience from a referral intensive care unit .
	manualset3
104573	3	402603	5	NULL	NULL	0	NULL	anterior resection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Management of postoperative peritonitis after anterior resection : experience from a referral intensive care unit .
	manualset3
104574	4	402603	5	NULL	NULL	0	NULL	experience 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Management of postoperative peritonitis after anterior resection : experience from a referral intensive care unit .
	manualset3
104575	5	402603	5	NULL	NULL	0	NULL	 referral intensive care unit	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Management of postoperative peritonitis after anterior resection : experience from a referral intensive care unit .
	manualset3
104576	1	402604	5	NULL	NULL	0	NULL	Management 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Management of the choked ureter in obstructive renal failure due to uric acid lithiasis .
	manualset3
104577	2	402604	5	NULL	NULL	0	NULL	choked ureter 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Management of the choked ureter in obstructive renal failure due to uric acid lithiasis .
	manualset3
104578	3	402604	5	NULL	NULL	0	NULL	obstructive renal failure	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Management of the choked ureter in obstructive renal failure due to uric acid lithiasis .
	manualset3
104579	4	402604	5	NULL	NULL	0	NULL	uric acid lithiasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Management of the choked ureter in obstructive renal failure due to uric acid lithiasis .
	manualset3
104580	1	402605	5	NULL	NULL	0	NULL	Management 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Management of uninvestigated and functional dyspepsia : a Working Party report for the World Congresses of Gastroenterology 1998 .
	manualset3
104581	2	402605	5	NULL	NULL	0	NULL	uninvestigated and functional dyspepsia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Management of uninvestigated and functional dyspepsia : a Working Party report for the World Congresses of Gastroenterology 1998 .
	manualset3
104582	3	402605	5	NULL	NULL	0	NULL	Working Party report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Management of uninvestigated and functional dyspepsia : a Working Party report for the World Congresses of Gastroenterology 1998 .
	manualset3
104583	4	402605	5	NULL	NULL	0	NULL	World Congresses of Gastroenterology	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Management of uninvestigated and functional dyspepsia : a Working Party report for the World Congresses of Gastroenterology 1998 .
	manualset3
104584	5	402605	5	NULL	NULL	0	NULL	1998 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Management of uninvestigated and functional dyspepsia : a Working Party report for the World Congresses of Gastroenterology 1998 .
	manualset3
104585	1	402606	5	NULL	NULL	0	NULL	Barodontology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Barodontology : clinical observations on etiology of dental problems in aviation medicine ) .
	manualset3
104586	2	402606	5	NULL	NULL	0	NULL	clinical observations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Barodontology : clinical observations on etiology of dental problems in aviation medicine ) .
	manualset3
104587	3	402606	5	NULL	NULL	0	NULL	etiology 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Barodontology : clinical observations on etiology of dental problems in aviation medicine ) .
	manualset3
104588	4	402606	5	NULL	NULL	0	NULL	dental problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Barodontology : clinical observations on etiology of dental problems in aviation medicine ) .
	manualset3
104589	5	402606	5	NULL	NULL	0	NULL	aviation medicine 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Barodontology : clinical observations on etiology of dental problems in aviation medicine ) .
	manualset3
104590	1	402607	5	NULL	NULL	0	NULL	JHA	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A JHA is a simple , time tested , and effective tool to assist in this analysis .
	manualset3
104591	2	402607	5	NULL	NULL	0	NULL	effective tool	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A JHA is a simple , time tested , and effective tool to assist in this analysis .
	manualset3
104592	3	402607	5	NULL	NULL	0	NULL	analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A JHA is a simple , time tested , and effective tool to assist in this analysis .
	manualset3
104593	1	402608	5	NULL	NULL	0	NULL	Management strategies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Management strategies for osteoarthritis , ankylosing spondylitis , and gouty arthritis .
	manualset3
104594	2	402608	5	NULL	NULL	0	NULL	osteoarthritis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Management strategies for osteoarthritis , ankylosing spondylitis , and gouty arthritis .
	manualset3
104595	3	402608	5	NULL	NULL	0	NULL	ankylosing spondylitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Management strategies for osteoarthritis , ankylosing spondylitis , and gouty arthritis .
	manualset3
104596	4	402608	5	NULL	NULL	0	NULL	gouty arthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Management strategies for osteoarthritis , ankylosing spondylitis , and gouty arthritis .
	manualset3
104597	1	402609	5	NULL	NULL	0	NULL	Managers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Managers of ambulatory surgery centers are philosophically in support of increased data collection to track medical events , but are wary of being swamped by paperwork , says a recent survey .
	manualset3
104598	2	402609	5	NULL	NULL	0	NULL	ambulatory surgery centers	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Managers of ambulatory surgery centers are philosophically in support of increased data collection to track medical events , but are wary of being swamped by paperwork , says a recent survey .
	manualset3
104599	3	402609	5	NULL	NULL	0	NULL	increased data collection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Managers of ambulatory surgery centers are philosophically in support of increased data collection to track medical events , but are wary of being swamped by paperwork , says a recent survey .
	manualset3
104600	4	402609	5	NULL	NULL	0	NULL	medical events	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Managers of ambulatory surgery centers are philosophically in support of increased data collection to track medical events , but are wary of being swamped by paperwork , says a recent survey .
	manualset3
104601	5	402609	5	NULL	NULL	0	NULL	paperwork 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Managers of ambulatory surgery centers are philosophically in support of increased data collection to track medical events , but are wary of being swamped by paperwork , says a recent survey .
	manualset3
104602	6	402609	5	NULL	NULL	0	NULL	recent survey	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Managers of ambulatory surgery centers are philosophically in support of increased data collection to track medical events , but are wary of being swamped by paperwork , says a recent survey .
	manualset3
104603	1	402610	5	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mandatory expression of hGSTA4 suppressed HNE-induced events .
	manualset3
104604	2	402610	5	NULL	NULL	0	NULL	hGSTA4 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mandatory expression of hGSTA4 suppressed HNE-induced events .
	manualset3
104605	3	402610	5	NULL	NULL	0	NULL	HNE-induced events	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mandatory expression of hGSTA4 suppressed HNE-induced events .
	manualset3
104606	1	402611	5	NULL	NULL	0	NULL	Manipulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Manipulation of direction of speech in a neuropsychiatric group .
	manualset3
104607	2	402611	5	NULL	NULL	0	NULL	direction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Manipulation of direction of speech in a neuropsychiatric group .
	manualset3
104608	3	402611	5	NULL	NULL	0	NULL	speech 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Manipulation of direction of speech in a neuropsychiatric group .
	manualset3
104609	4	402611	5	NULL	NULL	0	NULL	neuropsychiatric group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Manipulation of direction of speech in a neuropsychiatric group .
	manualset3
104610	1	402612	5	NULL	NULL	NULL	NULL	Manipulation 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Manipulation of doughnut focal spot by image inverting interferometry .
	manualset3
104611	2	402612	5	NULL	NULL	NULL	NULL	doughnut focal spot	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Manipulation of doughnut focal spot by image inverting interferometry .
	manualset3
104612	3	402612	5	NULL	NULL	0	NULL	image inverting interferometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Manipulation of doughnut focal spot by image inverting interferometry .
	manualset3
104613	1	402613	5	NULL	NULL	0	NULL	Mantle zones	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mantle zones and primary follicles contained more OKT4 + Leu-3a + and less OKT8 + cells than normally observed .
	manualset3
104614	2	402613	5	NULL	NULL	0	NULL	primary follicles 	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mantle zones and primary follicles contained more OKT4 + Leu-3a + and less OKT8 + cells than normally observed .
	manualset3
104615	3	402613	5	NULL	NULL	0	NULL	OKT4 + Leu-3a + cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mantle zones and primary follicles contained more OKT4 + Leu-3a + and less OKT8 + cells than normally observed .
	manualset3
104616	4	402613	5	NULL	NULL	0	NULL	OKT8 + cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mantle zones and primary follicles contained more OKT4 + Leu-3a + and less OKT8 + cells than normally observed .
	manualset3
104617	1	402614	5	NULL	NULL	0	NULL	Manufacture 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Manufacture and use of home made ophthalmoscopes : a 150th anniversary tribute to Helmholtz .
	manualset3
104618	2	402614	5	NULL	NULL	0	NULL	use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Manufacture and use of home made ophthalmoscopes : a 150th anniversary tribute to Helmholtz .
	manualset3
104619	3	402614	5	NULL	NULL	0	NULL	home made ophthalmoscopes	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Manufacture and use of home made ophthalmoscopes : a 150th anniversary tribute to Helmholtz .
	manualset3
104620	4	402614	5	NULL	NULL	0	NULL	150th anniversary tribute	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Manufacture and use of home made ophthalmoscopes : a 150th anniversary tribute to Helmholtz .
	manualset3
104621	5	402614	5	NULL	NULL	0	NULL	Helmholtz 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Manufacture and use of home made ophthalmoscopes : a 150th anniversary tribute to Helmholtz .
	manualset3
104797	1	402615	5	NULL	NULL	0	NULL	Manufactured nanomaterials ( MNs )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Manufactured nanomaterials ( MNs ) are commonly considered to be commercial products possessing at least one dimension in the size range of 10 ( -9 ) m to 10 ( -7 ) m. As particles in this size range represent the smaller fraction of colloidal particles characterized by dimensions of 10 ( -9 ) m to 10 ( -6 ) m , they differ from both molecular species and bulk particulate matter in the sense that they are unlikely to exhibit significant settling under normal gravitational conditions and they are also likely to exhibit significantly diminished diffusivities ( when compared to truly dissolved species ) in environmental media .
	manualset3
104798	2	402615	5	NULL	NULL	0	NULL	commercial products	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Manufactured nanomaterials ( MNs ) are commonly considered to be commercial products possessing at least one dimension in the size range of 10 ( -9 ) m to 10 ( -7 ) m. As particles in this size range represent the smaller fraction of colloidal particles characterized by dimensions of 10 ( -9 ) m to 10 ( -6 ) m , they differ from both molecular species and bulk particulate matter in the sense that they are unlikely to exhibit significant settling under normal gravitational conditions and they are also likely to exhibit significantly diminished diffusivities ( when compared to truly dissolved species ) in environmental media .
	manualset3
104799	3	402615	5	NULL	NULL	0	NULL	one dimension	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Manufactured nanomaterials ( MNs ) are commonly considered to be commercial products possessing at least one dimension in the size range of 10 ( -9 ) m to 10 ( -7 ) m. As particles in this size range represent the smaller fraction of colloidal particles characterized by dimensions of 10 ( -9 ) m to 10 ( -6 ) m , they differ from both molecular species and bulk particulate matter in the sense that they are unlikely to exhibit significant settling under normal gravitational conditions and they are also likely to exhibit significantly diminished diffusivities ( when compared to truly dissolved species ) in environmental media .
	manualset3
104800	4	402615	5	NULL	NULL	0	NULL	size range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Manufactured nanomaterials ( MNs ) are commonly considered to be commercial products possessing at least one dimension in the size range of 10 ( -9 ) m to 10 ( -7 ) m. As particles in this size range represent the smaller fraction of colloidal particles characterized by dimensions of 10 ( -9 ) m to 10 ( -6 ) m , they differ from both molecular species and bulk particulate matter in the sense that they are unlikely to exhibit significant settling under normal gravitational conditions and they are also likely to exhibit significantly diminished diffusivities ( when compared to truly dissolved species ) in environmental media .
	manualset3
104801	5	402615	5	NULL	NULL	0	NULL	10 ( -9 ) m to 10 ( -7 ) m	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Manufactured nanomaterials ( MNs ) are commonly considered to be commercial products possessing at least one dimension in the size range of 10 ( -9 ) m to 10 ( -7 ) m. As particles in this size range represent the smaller fraction of colloidal particles characterized by dimensions of 10 ( -9 ) m to 10 ( -6 ) m , they differ from both molecular species and bulk particulate matter in the sense that they are unlikely to exhibit significant settling under normal gravitational conditions and they are also likely to exhibit significantly diminished diffusivities ( when compared to truly dissolved species ) in environmental media .
	manualset3
104802	6	402615	5	NULL	NULL	0	NULL	particles	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Manufactured nanomaterials ( MNs ) are commonly considered to be commercial products possessing at least one dimension in the size range of 10 ( -9 ) m to 10 ( -7 ) m. As particles in this size range represent the smaller fraction of colloidal particles characterized by dimensions of 10 ( -9 ) m to 10 ( -6 ) m , they differ from both molecular species and bulk particulate matter in the sense that they are unlikely to exhibit significant settling under normal gravitational conditions and they are also likely to exhibit significantly diminished diffusivities ( when compared to truly dissolved species ) in environmental media .
	manualset3
104803	7	402615	5	NULL	NULL	0	NULL	size range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Manufactured nanomaterials ( MNs ) are commonly considered to be commercial products possessing at least one dimension in the size range of 10 ( -9 ) m to 10 ( -7 ) m. As particles in this size range represent the smaller fraction of colloidal particles characterized by dimensions of 10 ( -9 ) m to 10 ( -6 ) m , they differ from both molecular species and bulk particulate matter in the sense that they are unlikely to exhibit significant settling under normal gravitational conditions and they are also likely to exhibit significantly diminished diffusivities ( when compared to truly dissolved species ) in environmental media .
	manualset3
104804	8	402615	5	NULL	NULL	0	NULL	smaller fraction	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Manufactured nanomaterials ( MNs ) are commonly considered to be commercial products possessing at least one dimension in the size range of 10 ( -9 ) m to 10 ( -7 ) m. As particles in this size range represent the smaller fraction of colloidal particles characterized by dimensions of 10 ( -9 ) m to 10 ( -6 ) m , they differ from both molecular species and bulk particulate matter in the sense that they are unlikely to exhibit significant settling under normal gravitational conditions and they are also likely to exhibit significantly diminished diffusivities ( when compared to truly dissolved species ) in environmental media .
	manualset3
104805	9	402615	5	NULL	NULL	0	NULL	colloidal particles	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Manufactured nanomaterials ( MNs ) are commonly considered to be commercial products possessing at least one dimension in the size range of 10 ( -9 ) m to 10 ( -7 ) m. As particles in this size range represent the smaller fraction of colloidal particles characterized by dimensions of 10 ( -9 ) m to 10 ( -6 ) m , they differ from both molecular species and bulk particulate matter in the sense that they are unlikely to exhibit significant settling under normal gravitational conditions and they are also likely to exhibit significantly diminished diffusivities ( when compared to truly dissolved species ) in environmental media .
	manualset3
104806	10	402615	5	NULL	NULL	0	NULL	dimensions	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Manufactured nanomaterials ( MNs ) are commonly considered to be commercial products possessing at least one dimension in the size range of 10 ( -9 ) m to 10 ( -7 ) m. As particles in this size range represent the smaller fraction of colloidal particles characterized by dimensions of 10 ( -9 ) m to 10 ( -6 ) m , they differ from both molecular species and bulk particulate matter in the sense that they are unlikely to exhibit significant settling under normal gravitational conditions and they are also likely to exhibit significantly diminished diffusivities ( when compared to truly dissolved species ) in environmental media .
	manualset3
104807	11	402615	5	NULL	NULL	0	NULL	10 ( -9 ) m to 10 ( -6 ) m	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Manufactured nanomaterials ( MNs ) are commonly considered to be commercial products possessing at least one dimension in the size range of 10 ( -9 ) m to 10 ( -7 ) m. As particles in this size range represent the smaller fraction of colloidal particles characterized by dimensions of 10 ( -9 ) m to 10 ( -6 ) m , they differ from both molecular species and bulk particulate matter in the sense that they are unlikely to exhibit significant settling under normal gravitational conditions and they are also likely to exhibit significantly diminished diffusivities ( when compared to truly dissolved species ) in environmental media .
	manualset3
104808	12	402615	5	NULL	NULL	0	NULL	molecular species	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Manufactured nanomaterials ( MNs ) are commonly considered to be commercial products possessing at least one dimension in the size range of 10 ( -9 ) m to 10 ( -7 ) m. As particles in this size range represent the smaller fraction of colloidal particles characterized by dimensions of 10 ( -9 ) m to 10 ( -6 ) m , they differ from both molecular species and bulk particulate matter in the sense that they are unlikely to exhibit significant settling under normal gravitational conditions and they are also likely to exhibit significantly diminished diffusivities ( when compared to truly dissolved species ) in environmental media .
	manualset3
104809	13	402615	5	NULL	NULL	0	NULL	bulk particulate matter 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Manufactured nanomaterials ( MNs ) are commonly considered to be commercial products possessing at least one dimension in the size range of 10 ( -9 ) m to 10 ( -7 ) m. As particles in this size range represent the smaller fraction of colloidal particles characterized by dimensions of 10 ( -9 ) m to 10 ( -6 ) m , they differ from both molecular species and bulk particulate matter in the sense that they are unlikely to exhibit significant settling under normal gravitational conditions and they are also likely to exhibit significantly diminished diffusivities ( when compared to truly dissolved species ) in environmental media .
	manualset3
104810	14	402615	5	NULL	NULL	0	NULL	normal gravitational conditions	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Manufactured nanomaterials ( MNs ) are commonly considered to be commercial products possessing at least one dimension in the size range of 10 ( -9 ) m to 10 ( -7 ) m. As particles in this size range represent the smaller fraction of colloidal particles characterized by dimensions of 10 ( -9 ) m to 10 ( -6 ) m , they differ from both molecular species and bulk particulate matter in the sense that they are unlikely to exhibit significant settling under normal gravitational conditions and they are also likely to exhibit significantly diminished diffusivities ( when compared to truly dissolved species ) in environmental media .
	manualset3
104811	15	402615	5	NULL	NULL	0	NULL	diminished diffusivities	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Manufactured nanomaterials ( MNs ) are commonly considered to be commercial products possessing at least one dimension in the size range of 10 ( -9 ) m to 10 ( -7 ) m. As particles in this size range represent the smaller fraction of colloidal particles characterized by dimensions of 10 ( -9 ) m to 10 ( -6 ) m , they differ from both molecular species and bulk particulate matter in the sense that they are unlikely to exhibit significant settling under normal gravitational conditions and they are also likely to exhibit significantly diminished diffusivities ( when compared to truly dissolved species ) in environmental media .
	manualset3
104812	16	402615	5	NULL	NULL	0	NULL	truly dissolved species	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Manufactured nanomaterials ( MNs ) are commonly considered to be commercial products possessing at least one dimension in the size range of 10 ( -9 ) m to 10 ( -7 ) m. As particles in this size range represent the smaller fraction of colloidal particles characterized by dimensions of 10 ( -9 ) m to 10 ( -6 ) m , they differ from both molecular species and bulk particulate matter in the sense that they are unlikely to exhibit significant settling under normal gravitational conditions and they are also likely to exhibit significantly diminished diffusivities ( when compared to truly dissolved species ) in environmental media .
	manualset3
104813	17	402615	5	NULL	NULL	0	NULL	environmental media	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Manufactured nanomaterials ( MNs ) are commonly considered to be commercial products possessing at least one dimension in the size range of 10 ( -9 ) m to 10 ( -7 ) m. As particles in this size range represent the smaller fraction of colloidal particles characterized by dimensions of 10 ( -9 ) m to 10 ( -6 ) m , they differ from both molecular species and bulk particulate matter in the sense that they are unlikely to exhibit significant settling under normal gravitational conditions and they are also likely to exhibit significantly diminished diffusivities ( when compared to truly dissolved species ) in environmental media .
	manualset3
104814	1	402616	5	NULL	NULL	0	NULL	 Load-Matched group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A Load-Matched group received the same peak applied loads ( corresponding to +2100 at the medial diaphysis of the tibia ) and a Strain-Matched group received the same peak diaphyseal strains ( +1200 , requiring half the load ) as the young mice .
	manualset3
104815	2	402616	5	NULL	NULL	0	NULL	same peak applied loads	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A Load-Matched group received the same peak applied loads ( corresponding to +2100 at the medial diaphysis of the tibia ) and a Strain-Matched group received the same peak diaphyseal strains ( +1200 , requiring half the load ) as the young mice .
	manualset3
104816	3	402616	5	NULL	NULL	0	NULL	medial diaphysis 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A Load-Matched group received the same peak applied loads ( corresponding to +2100 at the medial diaphysis of the tibia ) and a Strain-Matched group received the same peak diaphyseal strains ( +1200 , requiring half the load ) as the young mice .
	manualset3
104817	4	402616	5	NULL	NULL	0	NULL	tibia	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A Load-Matched group received the same peak applied loads ( corresponding to +2100 at the medial diaphysis of the tibia ) and a Strain-Matched group received the same peak diaphyseal strains ( +1200 , requiring half the load ) as the young mice .
	manualset3
104818	5	402616	5	NULL	NULL	0	NULL	Strain-Matched group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A Load-Matched group received the same peak applied loads ( corresponding to +2100 at the medial diaphysis of the tibia ) and a Strain-Matched group received the same peak diaphyseal strains ( +1200 , requiring half the load ) as the young mice .
	manualset3
104819	6	402616	5	NULL	NULL	0	NULL	same peak diaphyseal strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A Load-Matched group received the same peak applied loads ( corresponding to +2100 at the medial diaphysis of the tibia ) and a Strain-Matched group received the same peak diaphyseal strains ( +1200 , requiring half the load ) as the young mice .
	manualset3
104820	7	402616	5	NULL	NULL	0	NULL	+1200	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A Load-Matched group received the same peak applied loads ( corresponding to +2100 at the medial diaphysis of the tibia ) and a Strain-Matched group received the same peak diaphyseal strains ( +1200 , requiring half the load ) as the young mice .
	manualset3
104821	8	402616	5	NULL	NULL	0	NULL	half	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A Load-Matched group received the same peak applied loads ( corresponding to +2100 at the medial diaphysis of the tibia ) and a Strain-Matched group received the same peak diaphyseal strains ( +1200 , requiring half the load ) as the young mice .
	manualset3
104822	9	402616	5	NULL	NULL	0	NULL	load	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A Load-Matched group received the same peak applied loads ( corresponding to +2100 at the medial diaphysis of the tibia ) and a Strain-Matched group received the same peak diaphyseal strains ( +1200 , requiring half the load ) as the young mice .
	manualset3
104823	10	402616	5	NULL	NULL	0	NULL	young mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A Load-Matched group received the same peak applied loads ( corresponding to +2100 at the medial diaphysis of the tibia ) and a Strain-Matched group received the same peak diaphyseal strains ( +1200 , requiring half the load ) as the young mice .
	manualset3
104824	1	402617	5	NULL	NULL	0	NULL	anticancer agents	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Many anticancer agents are known to induce apoptosis in cultured cells , but human solid tumor cells are often resistant to apoptosis induction .
	manualset3
104825	2	402617	5	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Many anticancer agents are known to induce apoptosis in cultured cells , but human solid tumor cells are often resistant to apoptosis induction .
	manualset3
104826	3	402617	5	NULL	NULL	0	NULL	cultured cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Many anticancer agents are known to induce apoptosis in cultured cells , but human solid tumor cells are often resistant to apoptosis induction .
	manualset3
104827	4	402617	5	NULL	NULL	0	NULL	human solid tumor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Many anticancer agents are known to induce apoptosis in cultured cells , but human solid tumor cells are often resistant to apoptosis induction .
	manualset3
104828	5	402617	5	NULL	NULL	0	NULL	apoptosis induction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Many anticancer agents are known to induce apoptosis in cultured cells , but human solid tumor cells are often resistant to apoptosis induction .
	manualset3
104829	1	402618	5	NULL	NULL	0	NULL	aphids	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Many aphids are known to engage in a trophic mutualism with ants , whereby the aphids secrete sugary-rich honeydew which is collected by the ants for food , and the ants , in exchange , protect the aphids against natural enemies .
	manualset3
104830	2	402618	5	NULL	NULL	0	NULL	trophic mutualism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Many aphids are known to engage in a trophic mutualism with ants , whereby the aphids secrete sugary-rich honeydew which is collected by the ants for food , and the ants , in exchange , protect the aphids against natural enemies .
	manualset3
104831	3	402618	5	NULL	NULL	0	NULL	ants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Many aphids are known to engage in a trophic mutualism with ants , whereby the aphids secrete sugary-rich honeydew which is collected by the ants for food , and the ants , in exchange , protect the aphids against natural enemies .
	manualset3
104832	4	402618	5	NULL	NULL	0	NULL	aphids	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Many aphids are known to engage in a trophic mutualism with ants , whereby the aphids secrete sugary-rich honeydew which is collected by the ants for food , and the ants , in exchange , protect the aphids against natural enemies .
	manualset3
104833	5	402618	5	NULL	NULL	0	NULL	sugary-rich honeydew	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Many aphids are known to engage in a trophic mutualism with ants , whereby the aphids secrete sugary-rich honeydew which is collected by the ants for food , and the ants , in exchange , protect the aphids against natural enemies .
	manualset3
104834	6	402618	5	NULL	NULL	0	NULL	ants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Many aphids are known to engage in a trophic mutualism with ants , whereby the aphids secrete sugary-rich honeydew which is collected by the ants for food , and the ants , in exchange , protect the aphids against natural enemies .
	manualset3
104835	7	402618	5	NULL	NULL	0	NULL	food	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Many aphids are known to engage in a trophic mutualism with ants , whereby the aphids secrete sugary-rich honeydew which is collected by the ants for food , and the ants , in exchange , protect the aphids against natural enemies .
	manualset3
104836	8	402618	5	NULL	NULL	0	NULL	ants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Many aphids are known to engage in a trophic mutualism with ants , whereby the aphids secrete sugary-rich honeydew which is collected by the ants for food , and the ants , in exchange , protect the aphids against natural enemies .
	manualset3
104837	9	402618	5	NULL	NULL	0	NULL	exchange	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many aphids are known to engage in a trophic mutualism with ants , whereby the aphids secrete sugary-rich honeydew which is collected by the ants for food , and the ants , in exchange , protect the aphids against natural enemies .
	manualset3
104838	10	402618	5	NULL	NULL	0	NULL	aphids	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Many aphids are known to engage in a trophic mutualism with ants , whereby the aphids secrete sugary-rich honeydew which is collected by the ants for food , and the ants , in exchange , protect the aphids against natural enemies .
	manualset3
104839	11	402618	5	NULL	NULL	0	NULL	natural enemies	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Many aphids are known to engage in a trophic mutualism with ants , whereby the aphids secrete sugary-rich honeydew which is collected by the ants for food , and the ants , in exchange , protect the aphids against natural enemies .
	manualset3
104840	1	402619	5	NULL	NULL	0	NULL	quiescence program	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Many aspects of the quiescence program as well as the mechanisms governing the entry and exit from quiescence remain poorly understood .
	manualset3
104841	2	402619	5	NULL	NULL	0	NULL	mechanisms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many aspects of the quiescence program as well as the mechanisms governing the entry and exit from quiescence remain poorly understood .
	manualset3
104842	3	402619	5	NULL	NULL	0	NULL	entry	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many aspects of the quiescence program as well as the mechanisms governing the entry and exit from quiescence remain poorly understood .
	manualset3
104843	4	402619	5	NULL	NULL	0	NULL	exit	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many aspects of the quiescence program as well as the mechanisms governing the entry and exit from quiescence remain poorly understood .
	manualset3
104844	5	402619	5	NULL	NULL	0	NULL	quiescence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Many aspects of the quiescence program as well as the mechanisms governing the entry and exit from quiescence remain poorly understood .
	manualset3
104845	1	402620	5	NULL	NULL	0	NULL	atopic dermatitis ( AD ) patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Many atopic dermatitis ( AD ) patients follow elimination diets for long periods of time because of true or -- even more often -- suspected food allergies or hypersensitivities .
	manualset3
104846	2	402620	5	NULL	NULL	0	NULL	elimination diets	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Many atopic dermatitis ( AD ) patients follow elimination diets for long periods of time because of true or -- even more often -- suspected food allergies or hypersensitivities .
	manualset3
104847	3	402620	5	NULL	NULL	0	NULL	long periods of time	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Many atopic dermatitis ( AD ) patients follow elimination diets for long periods of time because of true or -- even more often -- suspected food allergies or hypersensitivities .
	manualset3
104848	4	402620	5	NULL	NULL	0	NULL	suspected food allergies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Many atopic dermatitis ( AD ) patients follow elimination diets for long periods of time because of true or -- even more often -- suspected food allergies or hypersensitivities .
	manualset3
104849	5	402620	5	NULL	NULL	0	NULL	hypersensitivities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Many atopic dermatitis ( AD ) patients follow elimination diets for long periods of time because of true or -- even more often -- suspected food allergies or hypersensitivities .
	manualset3
104850	1	402621	5	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Many authors draw attention to the similarity of functioning of families with anorexia and bulimia .
	manualset3
104851	2	402621	5	NULL	NULL	0	NULL	attention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many authors draw attention to the similarity of functioning of families with anorexia and bulimia .
	manualset3
104852	3	402621	5	NULL	NULL	0	NULL	similarity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many authors draw attention to the similarity of functioning of families with anorexia and bulimia .
	manualset3
104853	4	402621	5	NULL	NULL	0	NULL	functioning of families	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many authors draw attention to the similarity of functioning of families with anorexia and bulimia .
	manualset3
104854	5	402621	5	NULL	NULL	0	NULL	anorexia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Many authors draw attention to the similarity of functioning of families with anorexia and bulimia .
	manualset3
104855	6	402621	5	NULL	NULL	0	NULL	bulimia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Many authors draw attention to the similarity of functioning of families with anorexia and bulimia .
	manualset3
104856	1	402622	5	NULL	NULL	0	NULL	congenital malformations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Many congenital malformations , such as cleft palate and neural tube defects , have a multifactorial origin involving both environmental and genetic factors .
	manualset3
104857	2	402622	5	NULL	NULL	0	NULL	cleft palate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Many congenital malformations , such as cleft palate and neural tube defects , have a multifactorial origin involving both environmental and genetic factors .
	manualset3
104858	3	402622	5	NULL	NULL	0	NULL	neural tube defects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Many congenital malformations , such as cleft palate and neural tube defects , have a multifactorial origin involving both environmental and genetic factors .
	manualset3
104859	4	402622	5	NULL	NULL	0	NULL	multifactorial origin	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many congenital malformations , such as cleft palate and neural tube defects , have a multifactorial origin involving both environmental and genetic factors .
	manualset3
104860	5	402622	5	NULL	NULL	0	NULL	environmental factors	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Many congenital malformations , such as cleft palate and neural tube defects , have a multifactorial origin involving both environmental and genetic factors .
	manualset3
104861	6	402622	5	NULL	NULL	NULL	NULL	genetic factors	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Many congenital malformations , such as cleft palate and neural tube defects , have a multifactorial origin involving both environmental and genetic factors .
	manualset3
104862	1	402623	5	NULL	NULL	0	NULL	discussions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many discussions and arguments about the techniques seem to underscore their true purpose , which is not `` simply to detoxify '' opiate-addicted patients but to initiate long-term management with naltrexone .
	manualset3
104863	2	402623	5	NULL	NULL	0	NULL	arguments 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many discussions and arguments about the techniques seem to underscore their true purpose , which is not `` simply to detoxify '' opiate-addicted patients but to initiate long-term management with naltrexone .
	manualset3
104864	3	402623	5	NULL	NULL	0	NULL	techniques 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Many discussions and arguments about the techniques seem to underscore their true purpose , which is not `` simply to detoxify '' opiate-addicted patients but to initiate long-term management with naltrexone .
	manualset3
104865	4	402623	5	NULL	NULL	0	NULL	purpose 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Many discussions and arguments about the techniques seem to underscore their true purpose , which is not `` simply to detoxify '' opiate-addicted patients but to initiate long-term management with naltrexone .
	manualset3
104866	5	402623	5	NULL	NULL	0	NULL	opiate-addicted patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Many discussions and arguments about the techniques seem to underscore their true purpose , which is not `` simply to detoxify '' opiate-addicted patients but to initiate long-term management with naltrexone .
	manualset3
104867	6	402623	5	NULL	NULL	0	NULL	long-term management 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Many discussions and arguments about the techniques seem to underscore their true purpose , which is not `` simply to detoxify '' opiate-addicted patients but to initiate long-term management with naltrexone .
	manualset3
104868	7	402623	5	NULL	NULL	0	NULL	naltrexone 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Many discussions and arguments about the techniques seem to underscore their true purpose , which is not `` simply to detoxify '' opiate-addicted patients but to initiate long-term management with naltrexone .
	manualset3
104869	1	402624	5	NULL	NULL	0	NULL	drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Many drugs can be used for adjuvant therapy of breast cancer , including anthracyclines , cyclophosphamide , 5-fluorouracil ( 5-fU ) and , recently , taxanes ( TXT ) have shown promising results .
	manualset3
104870	2	402624	5	NULL	NULL	0	NULL	adjuvant therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Many drugs can be used for adjuvant therapy of breast cancer , including anthracyclines , cyclophosphamide , 5-fluorouracil ( 5-fU ) and , recently , taxanes ( TXT ) have shown promising results .
	manualset3
104871	3	402624	5	NULL	NULL	0	NULL	breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Many drugs can be used for adjuvant therapy of breast cancer , including anthracyclines , cyclophosphamide , 5-fluorouracil ( 5-fU ) and , recently , taxanes ( TXT ) have shown promising results .
	manualset3
104872	4	402624	5	NULL	NULL	0	NULL	anthracyclines 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Many drugs can be used for adjuvant therapy of breast cancer , including anthracyclines , cyclophosphamide , 5-fluorouracil ( 5-fU ) and , recently , taxanes ( TXT ) have shown promising results .
	manualset3
104873	5	402624	5	NULL	NULL	0	NULL	 cyclophosphamide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Many drugs can be used for adjuvant therapy of breast cancer , including anthracyclines , cyclophosphamide , 5-fluorouracil ( 5-fU ) and , recently , taxanes ( TXT ) have shown promising results .
	manualset3
104874	6	402624	5	NULL	NULL	0	NULL	5-fluorouracil ( 5-fU )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Many drugs can be used for adjuvant therapy of breast cancer , including anthracyclines , cyclophosphamide , 5-fluorouracil ( 5-fU ) and , recently , taxanes ( TXT ) have shown promising results .
	manualset3
104875	7	402624	5	NULL	NULL	0	NULL	taxanes ( TXT ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Many drugs can be used for adjuvant therapy of breast cancer , including anthracyclines , cyclophosphamide , 5-fluorouracil ( 5-fU ) and , recently , taxanes ( TXT ) have shown promising results .
	manualset3
104876	8	402624	5	NULL	NULL	0	NULL	promising results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Many drugs can be used for adjuvant therapy of breast cancer , including anthracyclines , cyclophosphamide , 5-fluorouracil ( 5-fU ) and , recently , taxanes ( TXT ) have shown promising results .
	manualset3
104877	1	402625	5	NULL	NULL	0	NULL	Markov model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A Markov model assessing the effectiveness and cost-effectiveness of FOLFOX compared with FOLFIRI for the initial treatment of metastatic colorectal cancer .
	manualset3
104878	2	402625	5	NULL	NULL	0	NULL	FOLFOX 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A Markov model assessing the effectiveness and cost-effectiveness of FOLFOX compared with FOLFIRI for the initial treatment of metastatic colorectal cancer .
	manualset3
104879	3	402625	5	NULL	NULL	NULL	NULL	FOLFIRI 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A Markov model assessing the effectiveness and cost-effectiveness of FOLFOX compared with FOLFIRI for the initial treatment of metastatic colorectal cancer .
	manualset3
104907	4	402625	5	NULL	NULL	0	NULL	initial treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A Markov model assessing the effectiveness and cost-effectiveness of FOLFOX compared with FOLFIRI for the initial treatment of metastatic colorectal cancer .
	manualset3
104908	5	402625	5	NULL	NULL	0	NULL	metastatic colorectal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A Markov model assessing the effectiveness and cost-effectiveness of FOLFOX compared with FOLFIRI for the initial treatment of metastatic colorectal cancer .
	manualset3
104903	1	402626	5	NULL	NULL	0	NULL	genes encoding secreted and membrane proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Many genes encoding secreted and membrane proteins are included in the signature , suggesting the importance of tumor-microenvironment interactions during metastasis .
	manualset3
104904	2	402626	5	NULL	NULL	0	NULL	signature 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Many genes encoding secreted and membrane proteins are included in the signature , suggesting the importance of tumor-microenvironment interactions during metastasis .
	manualset3
104905	3	402626	5	NULL	NULL	0	NULL	tumor-microenvironment interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Many genes encoding secreted and membrane proteins are included in the signature , suggesting the importance of tumor-microenvironment interactions during metastasis .
	manualset3
104906	4	402626	5	NULL	NULL	0	NULL	metastasis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Many genes encoding secreted and membrane proteins are included in the signature , suggesting the importance of tumor-microenvironment interactions during metastasis .
	manualset3
104899	1	402627	5	NULL	NULL	0	NULL	health care facilities	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Many health care facilities , companies , and nonprofit organizations create home PEN patient education materials .
	manualset3
104900	2	402627	5	NULL	NULL	0	NULL	companies 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Many health care facilities , companies , and nonprofit organizations create home PEN patient education materials .
	manualset3
104901	3	402627	5	NULL	NULL	0	NULL	nonprofit organizations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Many health care facilities , companies , and nonprofit organizations create home PEN patient education materials .
	manualset3
104902	4	402627	5	NULL	NULL	0	NULL	home PEN patient education materials	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Many health care facilities , companies , and nonprofit organizations create home PEN patient education materials .
	manualset3
104892	1	402628	5	NULL	NULL	0	NULL	 indirect data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Many indirect data suggest that leukocytes might transfer signals to endothelial cells both through the release of active agents and adhesion to the endothelial cell surface .
	manualset3
104893	2	402628	5	NULL	NULL	0	NULL	leukocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Many indirect data suggest that leukocytes might transfer signals to endothelial cells both through the release of active agents and adhesion to the endothelial cell surface .
	manualset3
104894	3	402628	5	NULL	NULL	0	NULL	transfer signals 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Many indirect data suggest that leukocytes might transfer signals to endothelial cells both through the release of active agents and adhesion to the endothelial cell surface .
	manualset3
104895	4	402628	5	NULL	NULL	0	NULL	endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Many indirect data suggest that leukocytes might transfer signals to endothelial cells both through the release of active agents and adhesion to the endothelial cell surface .
	manualset3
104896	5	402628	5	NULL	NULL	0	NULL	 active agents 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Many indirect data suggest that leukocytes might transfer signals to endothelial cells both through the release of active agents and adhesion to the endothelial cell surface .
	manualset3
104897	6	402628	5	NULL	NULL	0	NULL	adhesion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Many indirect data suggest that leukocytes might transfer signals to endothelial cells both through the release of active agents and adhesion to the endothelial cell surface .
	manualset3
104898	7	402628	5	NULL	NULL	0	NULL	endothelial cell surface	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Many indirect data suggest that leukocytes might transfer signals to endothelial cells both through the release of active agents and adhesion to the endothelial cell surface .
	manualset3
104886	1	402629	5	NULL	NULL	0	NULL	lines of evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Many lines of evidence indicate that GABA and GABA ( A ) receptors make important contributions to human sleep regulation .
	manualset3
104887	2	402629	5	NULL	NULL	0	NULL	GABA 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Many lines of evidence indicate that GABA and GABA ( A ) receptors make important contributions to human sleep regulation .
	manualset3
104888	3	402629	5	NULL	NULL	0	NULL	GABA ( A ) receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Many lines of evidence indicate that GABA and GABA ( A ) receptors make important contributions to human sleep regulation .
	manualset3
104889	4	402629	5	NULL	NULL	0	NULL	important contributions 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Many lines of evidence indicate that GABA and GABA ( A ) receptors make important contributions to human sleep regulation .
	manualset3
104890	5	402629	5	NULL	NULL	0	NULL	human	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Many lines of evidence indicate that GABA and GABA ( A ) receptors make important contributions to human sleep regulation .
	manualset3
104891	6	402629	5	NULL	NULL	0	NULL	sleep regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Many lines of evidence indicate that GABA and GABA ( A ) receptors make important contributions to human sleep regulation .
	manualset3
104880	1	402630	5	NULL	NULL	0	NULL	lncRNAs 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Many lncRNAs regulate gene expression through formation of epigenetic ribonucleoprotein complexes , including TUG1 and MEG3 .
	manualset3
104881	2	402630	5	NULL	NULL	0	NULL	gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Many lncRNAs regulate gene expression through formation of epigenetic ribonucleoprotein complexes , including TUG1 and MEG3 .
	manualset3
104882	3	402630	5	NULL	NULL	0	NULL	formation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many lncRNAs regulate gene expression through formation of epigenetic ribonucleoprotein complexes , including TUG1 and MEG3 .
	manualset3
104883	4	402630	5	NULL	NULL	0	NULL	epigenetic ribonucleoprotein complexes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Many lncRNAs regulate gene expression through formation of epigenetic ribonucleoprotein complexes , including TUG1 and MEG3 .
	manualset3
104884	5	402630	5	NULL	NULL	0	NULL	TUG1 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Many lncRNAs regulate gene expression through formation of epigenetic ribonucleoprotein complexes , including TUG1 and MEG3 .
	manualset3
104885	6	402630	5	NULL	NULL	0	NULL	MEG3 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Many lncRNAs regulate gene expression through formation of epigenetic ribonucleoprotein complexes , including TUG1 and MEG3 .
	manualset3
104909	1	402631	5	NULL	NULL	0	NULL	methods 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many methods of reconstruction of the nipple have been described in the last few years , but none are completely satisfactory .
	manualset3
104910	2	402631	5	NULL	NULL	0	NULL	reconstruction 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Many methods of reconstruction of the nipple have been described in the last few years , but none are completely satisfactory .
	manualset3
104911	3	402631	5	NULL	NULL	0	NULL	nipple 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Many methods of reconstruction of the nipple have been described in the last few years , but none are completely satisfactory .
	manualset3
104912	4	402631	5	NULL	NULL	0	NULL	last few years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Many methods of reconstruction of the nipple have been described in the last few years , but none are completely satisfactory .
	manualset3
104913	1	402632	5	NULL	NULL	0	NULL	Markov model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A Markov model simulated the progression of 20 - and 40-yr-old close contacts of active TB cases over 20 yrs .
	manualset3
104914	2	402632	5	NULL	NULL	0	NULL	progression 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A Markov model simulated the progression of 20 - and 40-yr-old close contacts of active TB cases over 20 yrs .
	manualset3
104915	3	402632	5	NULL	NULL	0	NULL	20 - yr-old close contacts 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A Markov model simulated the progression of 20 - and 40-yr-old close contacts of active TB cases over 20 yrs .
	manualset3
104916	4	402632	5	NULL	NULL	0	NULL	40-yr-old close contacts	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A Markov model simulated the progression of 20 - and 40-yr-old close contacts of active TB cases over 20 yrs .
	manualset3
104917	5	402632	5	NULL	NULL	0	NULL	active TB cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A Markov model simulated the progression of 20 - and 40-yr-old close contacts of active TB cases over 20 yrs .
	manualset3
104918	6	402632	5	NULL	NULL	0	NULL	20 yrs	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	A Markov model simulated the progression of 20 - and 40-yr-old close contacts of active TB cases over 20 yrs .
	manualset3
104919	1	402633	5	NULL	NULL	0	NULL	microalgae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Many microalgae accumulate oils , particularly under conditions limiting to growth , and thus have gained renewed attention as a potentially sustainable feedstock for biofuel production .
	manualset3
104920	2	402633	5	NULL	NULL	0	NULL	oils 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Many microalgae accumulate oils , particularly under conditions limiting to growth , and thus have gained renewed attention as a potentially sustainable feedstock for biofuel production .
	manualset3
104921	3	402633	5	NULL	NULL	0	NULL	conditions 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Many microalgae accumulate oils , particularly under conditions limiting to growth , and thus have gained renewed attention as a potentially sustainable feedstock for biofuel production .
	manualset3
104922	4	402633	5	NULL	NULL	0	NULL	growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Many microalgae accumulate oils , particularly under conditions limiting to growth , and thus have gained renewed attention as a potentially sustainable feedstock for biofuel production .
	manualset3
104923	5	402633	5	NULL	NULL	0	NULL	renewed attention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many microalgae accumulate oils , particularly under conditions limiting to growth , and thus have gained renewed attention as a potentially sustainable feedstock for biofuel production .
	manualset3
104924	6	402633	5	NULL	NULL	0	NULL	potentially sustainable feedstock	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Many microalgae accumulate oils , particularly under conditions limiting to growth , and thus have gained renewed attention as a potentially sustainable feedstock for biofuel production .
	manualset3
104925	7	402633	5	NULL	NULL	0	NULL	biofuel production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many microalgae accumulate oils , particularly under conditions limiting to growth , and thus have gained renewed attention as a potentially sustainable feedstock for biofuel production .
	manualset3
104926	1	402634	5	NULL	NULL	0	NULL	neurons 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Many neurons of the central and peripheral nervous systems display multiple high voltage-activated ( HVA ) Ca2 + currents , often classified as L - , N - , P - , Q , and R-type .
	manualset3
104927	2	402634	5	NULL	NULL	NULL	NULL	central and peripheral nervous systems	AnatomicalPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Many neurons of the central and peripheral nervous systems display multiple high voltage-activated ( HVA ) Ca2 + currents , often classified as L - , N - , P - , Q , and R-type .
	manualset3
105920	3	402634	5	NULL	NULL	NULL	NULL	high voltage-activated ( HVA ) Ca2 + currents	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Many neurons of the central and peripheral nervous systems display multiple high voltage-activated ( HVA ) Ca2 + currents , often classified as L - , N - , P - , Q , and R-type .
	manualset3
105921	4	402634	5	NULL	NULL	NULL	NULL	L - type	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Many neurons of the central and peripheral nervous systems display multiple high voltage-activated ( HVA ) Ca2 + currents , often classified as L - , N - , P - , Q , and R-type .
	manualset3
105922	5	402634	5	NULL	NULL	NULL	NULL	N - type	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Many neurons of the central and peripheral nervous systems display multiple high voltage-activated ( HVA ) Ca2 + currents , often classified as L - , N - , P - , Q , and R-type .
	manualset3
105923	6	402634	5	NULL	NULL	0	NULL	P - type	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many neurons of the central and peripheral nervous systems display multiple high voltage-activated ( HVA ) Ca2 + currents , often classified as L - , N - , P - , Q , and R-type .
	manualset3
105924	7	402634	5	NULL	NULL	0	NULL	Q - type	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many neurons of the central and peripheral nervous systems display multiple high voltage-activated ( HVA ) Ca2 + currents , often classified as L - , N - , P - , Q , and R-type .
	manualset3
105925	7	402634	5	NULL	NULL	0	NULL	Q - type	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many neurons of the central and peripheral nervous systems display multiple high voltage-activated ( HVA ) Ca2 + currents , often classified as L - , N - , P - , Q , and R-type .
	manualset3
105926	8	402634	5	NULL	NULL	0	NULL	R-type	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many neurons of the central and peripheral nervous systems display multiple high voltage-activated ( HVA ) Ca2 + currents , often classified as L - , N - , P - , Q , and R-type .
	manualset3
105927	1	402635	5	NULL	NULL	0	NULL	cysts 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Many of the cysts were lined with a benign mucinous epithelium of the endocervical type , and solid areas contained a proliferation of granulosa cells .
	manualset3
105928	2	402635	5	NULL	NULL	0	NULL	benign mucinous epithelium	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Many of the cysts were lined with a benign mucinous epithelium of the endocervical type , and solid areas contained a proliferation of granulosa cells .
	manualset3
105929	3	402635	5	NULL	NULL	0	NULL	endocervical type 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Many of the cysts were lined with a benign mucinous epithelium of the endocervical type , and solid areas contained a proliferation of granulosa cells .
	manualset3
105930	4	402635	5	NULL	NULL	0	NULL	solid areas	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Many of the cysts were lined with a benign mucinous epithelium of the endocervical type , and solid areas contained a proliferation of granulosa cells .
	manualset3
105931	5	402635	5	NULL	NULL	NULL	NULL	proliferation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Many of the cysts were lined with a benign mucinous epithelium of the endocervical type , and solid areas contained a proliferation of granulosa cells .
	manualset3
105933	6	402635	5	NULL	NULL	0	NULL	granulosa cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Many of the cysts were lined with a benign mucinous epithelium of the endocervical type , and solid areas contained a proliferation of granulosa cells .
	manualset3
105936	1	402636	5	NULL	NULL	0	NULL	daily survival tactics	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many of the daily survival tactics employed by runaways put them at risk for a variety of medical problems , including sexually transmitted diseases , hepatitis , tuberculosis , trauma , accidents , and HIV infection .
	manualset3
105937	2	402636	5	NULL	NULL	0	NULL	runaways	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Many of the daily survival tactics employed by runaways put them at risk for a variety of medical problems , including sexually transmitted diseases , hepatitis , tuberculosis , trauma , accidents , and HIV infection .
	manualset3
105939	3	402636	5	NULL	NULL	0	NULL	risk	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many of the daily survival tactics employed by runaways put them at risk for a variety of medical problems , including sexually transmitted diseases , hepatitis , tuberculosis , trauma , accidents , and HIV infection .
	manualset3
105940	4	402636	5	NULL	NULL	0	NULL	medical problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Many of the daily survival tactics employed by runaways put them at risk for a variety of medical problems , including sexually transmitted diseases , hepatitis , tuberculosis , trauma , accidents , and HIV infection .
	manualset3
105942	5	402636	5	NULL	NULL	0	NULL	sexually transmitted diseases 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Many of the daily survival tactics employed by runaways put them at risk for a variety of medical problems , including sexually transmitted diseases , hepatitis , tuberculosis , trauma , accidents , and HIV infection .
	manualset3
105944	6	402636	5	NULL	NULL	0	NULL	hepatitis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Many of the daily survival tactics employed by runaways put them at risk for a variety of medical problems , including sexually transmitted diseases , hepatitis , tuberculosis , trauma , accidents , and HIV infection .
	manualset3
105945	7	402636	5	NULL	NULL	0	NULL	tuberculosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Many of the daily survival tactics employed by runaways put them at risk for a variety of medical problems , including sexually transmitted diseases , hepatitis , tuberculosis , trauma , accidents , and HIV infection .
	manualset3
105947	8	402636	5	NULL	NULL	0	NULL	trauma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Many of the daily survival tactics employed by runaways put them at risk for a variety of medical problems , including sexually transmitted diseases , hepatitis , tuberculosis , trauma , accidents , and HIV infection .
	manualset3
105948	9	402636	5	NULL	NULL	0	NULL	accidents 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Many of the daily survival tactics employed by runaways put them at risk for a variety of medical problems , including sexually transmitted diseases , hepatitis , tuberculosis , trauma , accidents , and HIV infection .
	manualset3
105950	10	402636	5	NULL	NULL	0	NULL	HIV infection	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Many of the daily survival tactics employed by runaways put them at risk for a variety of medical problems , including sexually transmitted diseases , hepatitis , tuberculosis , trauma , accidents , and HIV infection .
	manualset3
105952	1	402637	5	NULL	NULL	NULL	NULL	inherent problems	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Many of the inherent problems associated with older sorbents have been overcome by designing sorbents with improved biocompatibility and potential for removing molecules beyond the limits of conventional dialysis membranes .
	manualset3
105953	2	402637	5	NULL	NULL	0	NULL	older sorbents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Many of the inherent problems associated with older sorbents have been overcome by designing sorbents with improved biocompatibility and potential for removing molecules beyond the limits of conventional dialysis membranes .
	manualset3
105954	3	402637	5	NULL	NULL	0	NULL	sorbents 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Many of the inherent problems associated with older sorbents have been overcome by designing sorbents with improved biocompatibility and potential for removing molecules beyond the limits of conventional dialysis membranes .
	manualset3
105955	4	402637	5	NULL	NULL	0	NULL	improved biocompatibility	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Many of the inherent problems associated with older sorbents have been overcome by designing sorbents with improved biocompatibility and potential for removing molecules beyond the limits of conventional dialysis membranes .
	manualset3
105956	5	402637	5	NULL	NULL	0	NULL	potential 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many of the inherent problems associated with older sorbents have been overcome by designing sorbents with improved biocompatibility and potential for removing molecules beyond the limits of conventional dialysis membranes .
	manualset3
105957	6	402637	5	NULL	NULL	0	NULL	molecules 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Many of the inherent problems associated with older sorbents have been overcome by designing sorbents with improved biocompatibility and potential for removing molecules beyond the limits of conventional dialysis membranes .
	manualset3
105958	7	402637	5	NULL	NULL	0	NULL	conventional dialysis membranes	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Many of the inherent problems associated with older sorbents have been overcome by designing sorbents with improved biocompatibility and potential for removing molecules beyond the limits of conventional dialysis membranes .
	manualset3
105959	1	402638	5	NULL	NULL	0	NULL	neuronal ligand-receptor interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Many of these are involved in neuronal ligand-receptor interactions and signaling cascades for activity dependent gene expression .
	manualset3
105960	2	402638	5	NULL	NULL	0	NULL	signaling cascades	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Many of these are involved in neuronal ligand-receptor interactions and signaling cascades for activity dependent gene expression .
	manualset3
105961	3	402638	5	NULL	NULL	0	NULL	activity dependent gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Many of these are involved in neuronal ligand-receptor interactions and signaling cascades for activity dependent gene expression .
	manualset3
105962	1	402639	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Many patients with HIV infection have comorbid substance use disorders .
	manualset3
105963	2	402639	5	NULL	NULL	0	NULL	HIV infection	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Many patients with HIV infection have comorbid substance use disorders .
	manualset3
105964	3	402639	5	NULL	NULL	0	NULL	comorbid substance use disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Many patients with HIV infection have comorbid substance use disorders .
	manualset3
105965	1	402640	5	NULL	NULL	0	NULL	programs	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many programs struggle to ensure that students are given an adequate exposure to and appreciation of ethical and professional conduct issues .
	manualset3
105966	2	402640	5	NULL	NULL	0	NULL	students 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Many programs struggle to ensure that students are given an adequate exposure to and appreciation of ethical and professional conduct issues .
	manualset3
105967	3	402640	5	NULL	NULL	0	NULL	adequate exposure 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many programs struggle to ensure that students are given an adequate exposure to and appreciation of ethical and professional conduct issues .
	manualset3
105968	4	402640	5	NULL	NULL	0	NULL	appreciation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many programs struggle to ensure that students are given an adequate exposure to and appreciation of ethical and professional conduct issues .
	manualset3
105969	5	402640	5	NULL	NULL	0	NULL	ethical conduct issues	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Many programs struggle to ensure that students are given an adequate exposure to and appreciation of ethical and professional conduct issues .
	manualset3
105970	6	402640	5	NULL	NULL	0	NULL	professional conduct issues	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Many programs struggle to ensure that students are given an adequate exposure to and appreciation of ethical and professional conduct issues .
	manualset3
105971	1	402641	5	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Many studies involving low-level laser therapy have shown that the healing process is enhanced by such therapy .
	manualset3
105972	2	402641	5	NULL	NULL	0	NULL	low-level laser therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Many studies involving low-level laser therapy have shown that the healing process is enhanced by such therapy .
	manualset3
105973	3	402641	5	NULL	NULL	0	NULL	healing process	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Many studies involving low-level laser therapy have shown that the healing process is enhanced by such therapy .
	manualset3
105974	4	402641	5	NULL	NULL	0	NULL	therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Many studies involving low-level laser therapy have shown that the healing process is enhanced by such therapy .
	manualset3
105975	1	402642	5	NULL	NULL	0	NULL	Islam 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Many think that Islam prevents them from divorce and allows their husbands to abuse them .
	manualset3
105976	2	402642	5	NULL	NULL	0	NULL	divorce 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many think that Islam prevents them from divorce and allows their husbands to abuse them .
	manualset3
105977	3	402642	5	NULL	NULL	0	NULL	husbands 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Many think that Islam prevents them from divorce and allows their husbands to abuse them .
	manualset3
105979	1	402643	5	NULL	NULL	0	NULL	viruses 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Many viruses and bacterial toxins use endocytic pathways to invade the host mammalian cells , and some of these pathogens have the ability to facilitate their endosomal escape into the cytosol by pH-induced alteration in their component proteins that leads to the disruption of the endosomal membranes and the eventual membrane fusions .
	manualset3
105980	2	402643	5	NULL	NULL	0	NULL	bacterial toxins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Many viruses and bacterial toxins use endocytic pathways to invade the host mammalian cells , and some of these pathogens have the ability to facilitate their endosomal escape into the cytosol by pH-induced alteration in their component proteins that leads to the disruption of the endosomal membranes and the eventual membrane fusions .
	manualset3
105981	3	402643	5	NULL	NULL	0	NULL	endocytic pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Many viruses and bacterial toxins use endocytic pathways to invade the host mammalian cells , and some of these pathogens have the ability to facilitate their endosomal escape into the cytosol by pH-induced alteration in their component proteins that leads to the disruption of the endosomal membranes and the eventual membrane fusions .
	manualset3
105982	4	402643	5	NULL	NULL	0	NULL	host mammalian cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Many viruses and bacterial toxins use endocytic pathways to invade the host mammalian cells , and some of these pathogens have the ability to facilitate their endosomal escape into the cytosol by pH-induced alteration in their component proteins that leads to the disruption of the endosomal membranes and the eventual membrane fusions .
	manualset3
105983	5	402643	5	NULL	NULL	0	NULL	pathogens 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Many viruses and bacterial toxins use endocytic pathways to invade the host mammalian cells , and some of these pathogens have the ability to facilitate their endosomal escape into the cytosol by pH-induced alteration in their component proteins that leads to the disruption of the endosomal membranes and the eventual membrane fusions .
	manualset3
105984	6	402643	5	NULL	NULL	0	NULL	endosomal escape	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many viruses and bacterial toxins use endocytic pathways to invade the host mammalian cells , and some of these pathogens have the ability to facilitate their endosomal escape into the cytosol by pH-induced alteration in their component proteins that leads to the disruption of the endosomal membranes and the eventual membrane fusions .
	manualset3
105985	7	402643	5	NULL	NULL	0	NULL	cytosol 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Many viruses and bacterial toxins use endocytic pathways to invade the host mammalian cells , and some of these pathogens have the ability to facilitate their endosomal escape into the cytosol by pH-induced alteration in their component proteins that leads to the disruption of the endosomal membranes and the eventual membrane fusions .
	manualset3
105986	8	402643	5	NULL	NULL	0	NULL	pH-induced alteration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many viruses and bacterial toxins use endocytic pathways to invade the host mammalian cells , and some of these pathogens have the ability to facilitate their endosomal escape into the cytosol by pH-induced alteration in their component proteins that leads to the disruption of the endosomal membranes and the eventual membrane fusions .
	manualset3
105989	9	402643	5	NULL	NULL	0	NULL	component proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Many viruses and bacterial toxins use endocytic pathways to invade the host mammalian cells , and some of these pathogens have the ability to facilitate their endosomal escape into the cytosol by pH-induced alteration in their component proteins that leads to the disruption of the endosomal membranes and the eventual membrane fusions .
	manualset3
105990	10	402643	5	NULL	NULL	0	NULL	disruption 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many viruses and bacterial toxins use endocytic pathways to invade the host mammalian cells , and some of these pathogens have the ability to facilitate their endosomal escape into the cytosol by pH-induced alteration in their component proteins that leads to the disruption of the endosomal membranes and the eventual membrane fusions .
	manualset3
105992	11	402643	5	NULL	NULL	0	NULL	endosomal membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Many viruses and bacterial toxins use endocytic pathways to invade the host mammalian cells , and some of these pathogens have the ability to facilitate their endosomal escape into the cytosol by pH-induced alteration in their component proteins that leads to the disruption of the endosomal membranes and the eventual membrane fusions .
	manualset3
105993	12	402643	5	NULL	NULL	0	NULL	eventual membrane fusions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Many viruses and bacterial toxins use endocytic pathways to invade the host mammalian cells , and some of these pathogens have the ability to facilitate their endosomal escape into the cytosol by pH-induced alteration in their component proteins that leads to the disruption of the endosomal membranes and the eventual membrane fusions .
	manualset3
105996	1	402644	5	NULL	NULL	0	NULL	war casualties	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Many war casualties are women and children .
	manualset3
105997	2	402644	5	NULL	NULL	0	NULL	women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Many war casualties are women and children .
	manualset3
105998	3	402644	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Many war casualties are women and children .
	manualset3
105999	1	402645	5	NULL	NULL	0	NULL	homogenates 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Many were also present in homogenates of host-tissue , but biochemical evidence is presented which indicates that all enzymes detected in extracts from M. leprae were authentic bacterial enzymes .
	manualset3
106000	2	402645	5	NULL	NULL	0	NULL	host-tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Many were also present in homogenates of host-tissue , but biochemical evidence is presented which indicates that all enzymes detected in extracts from M. leprae were authentic bacterial enzymes .
	manualset3
106001	3	402645	5	NULL	NULL	0	NULL	biochemical evidence	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Many were also present in homogenates of host-tissue , but biochemical evidence is presented which indicates that all enzymes detected in extracts from M. leprae were authentic bacterial enzymes .
	manualset3
106003	4	402645	5	NULL	NULL	0	NULL	enzymes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Many were also present in homogenates of host-tissue , but biochemical evidence is presented which indicates that all enzymes detected in extracts from M. leprae were authentic bacterial enzymes .
	manualset3
106005	5	402645	5	NULL	NULL	0	NULL	extracts 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Many were also present in homogenates of host-tissue , but biochemical evidence is presented which indicates that all enzymes detected in extracts from M. leprae were authentic bacterial enzymes .
	manualset3
106006	6	402645	5	NULL	NULL	0	NULL	M. leprae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Many were also present in homogenates of host-tissue , but biochemical evidence is presented which indicates that all enzymes detected in extracts from M. leprae were authentic bacterial enzymes .
	manualset3
106008	7	402645	5	NULL	NULL	0	NULL	authentic bacterial enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Many were also present in homogenates of host-tissue , but biochemical evidence is presented which indicates that all enzymes detected in extracts from M. leprae were authentic bacterial enzymes .
	manualset3
106010	1	402646	5	NULL	NULL	0	NULL	yeast strains 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Many yeast strains undergo a developmental transition in which cells of one mating type differentiate into a distinct cell type by a programmed genetic rearrangement at the MAT locus .
	manualset3
106012	2	402646	5	NULL	NULL	0	NULL	developmental transition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Many yeast strains undergo a developmental transition in which cells of one mating type differentiate into a distinct cell type by a programmed genetic rearrangement at the MAT locus .
	manualset3
106015	3	402646	5	NULL	NULL	0	NULL	cells of one mating type	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Many yeast strains undergo a developmental transition in which cells of one mating type differentiate into a distinct cell type by a programmed genetic rearrangement at the MAT locus .
	manualset3
106016	4	402646	5	NULL	NULL	0	NULL	distinct cell type	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Many yeast strains undergo a developmental transition in which cells of one mating type differentiate into a distinct cell type by a programmed genetic rearrangement at the MAT locus .
	manualset3
106017	5	402646	5	NULL	NULL	NULL	NULL	programmed genetic rearrangement	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Many yeast strains undergo a developmental transition in which cells of one mating type differentiate into a distinct cell type by a programmed genetic rearrangement at the MAT locus .
	manualset3
106018	6	402646	5	NULL	NULL	0	NULL	MAT locus	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Many yeast strains undergo a developmental transition in which cells of one mating type differentiate into a distinct cell type by a programmed genetic rearrangement at the MAT locus .
	manualset3
106019	1	402647	5	NULL	NULL	NULL	NULL	dystrophin gene recombinants	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mapping dystrophin gene recombinants in Greek DMD/BMD families : low recombination frequencies in the STR region .
	manualset3
106023	2	402647	5	NULL	NULL	0	NULL	Greek DMD/BMD families	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mapping dystrophin gene recombinants in Greek DMD/BMD families : low recombination frequencies in the STR region .
	manualset3
106024	3	402647	5	NULL	NULL	0	NULL	low recombination frequencies	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mapping dystrophin gene recombinants in Greek DMD/BMD families : low recombination frequencies in the STR region .
	manualset3
106025	4	402647	5	NULL	NULL	0	NULL	STR region 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Mapping dystrophin gene recombinants in Greek DMD/BMD families : low recombination frequencies in the STR region .
	manualset3
106029	1	402648	5	NULL	NULL	NULL	NULL	iron binding sites	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mapping iron binding sites on human frataxin : implications for cluster assembly on the ISU Fe-S cluster scaffold protein .
	manualset3
106031	2	402648	5	NULL	NULL	NULL	NULL	human frataxin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mapping iron binding sites on human frataxin : implications for cluster assembly on the ISU Fe-S cluster scaffold protein .
	manualset3
106034	3	402648	5	NULL	NULL	0	NULL	cluster assembly	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mapping iron binding sites on human frataxin : implications for cluster assembly on the ISU Fe-S cluster scaffold protein .
	manualset3
106035	4	402648	5	NULL	NULL	0	NULL	 ISU Fe-S cluster scaffold protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mapping iron binding sites on human frataxin : implications for cluster assembly on the ISU Fe-S cluster scaffold protein .
	manualset3
106036	1	402649	5	NULL	NULL	0	NULL	neurocan binding site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mapping of a defined neurocan binding site to distinct domains of tenascin-C .
	manualset3
106039	2	402649	5	NULL	NULL	0	NULL	distinct domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mapping of a defined neurocan binding site to distinct domains of tenascin-C .
	manualset3
106040	3	402649	5	NULL	NULL	0	NULL	tenascin-C	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mapping of a defined neurocan binding site to distinct domains of tenascin-C .
	manualset3
106046	1	402650	5	NULL	NULL	0	NULL	active site polarity	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mapping the active site polarity in structures of endothelial nitric oxide synthase heme domain complexed with isothioureas .
	manualset3
106047	2	402650	5	NULL	NULL	0	NULL	structures 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mapping the active site polarity in structures of endothelial nitric oxide synthase heme domain complexed with isothioureas .
	manualset3
106048	3	402650	5	NULL	NULL	0	NULL	endothelial nitric oxide synthase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mapping the active site polarity in structures of endothelial nitric oxide synthase heme domain complexed with isothioureas .
	manualset3
106050	4	402650	5	NULL	NULL	0	NULL	heme domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mapping the active site polarity in structures of endothelial nitric oxide synthase heme domain complexed with isothioureas .
	manualset3
106055	5	402650	5	NULL	NULL	0	NULL	isothioureas 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Mapping the active site polarity in structures of endothelial nitric oxide synthase heme domain complexed with isothioureas .
	manualset3
106056	1	402651	5	NULL	NULL	0	NULL	distribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mapping the distribution of the interstitial telomeric ( TTAGGG ) n sequences in eight species of Brazilian marsupials ( Didelphidae ) by FISH and the correlation with constitutive heterochromatin .
	manualset3
106057	2	402651	5	NULL	NULL	0	NULL	interstitial telomeric ( TTAGGG ) n sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Mapping the distribution of the interstitial telomeric ( TTAGGG ) n sequences in eight species of Brazilian marsupials ( Didelphidae ) by FISH and the correlation with constitutive heterochromatin .
	manualset3
106058	3	402651	5	NULL	NULL	0	NULL	eight species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mapping the distribution of the interstitial telomeric ( TTAGGG ) n sequences in eight species of Brazilian marsupials ( Didelphidae ) by FISH and the correlation with constitutive heterochromatin .
	manualset3
106059	4	402651	5	NULL	NULL	0	NULL	Brazilian marsupials ( Didelphidae )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mapping the distribution of the interstitial telomeric ( TTAGGG ) n sequences in eight species of Brazilian marsupials ( Didelphidae ) by FISH and the correlation with constitutive heterochromatin .
	manualset3
106060	5	402651	5	NULL	NULL	0	NULL	FISH 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mapping the distribution of the interstitial telomeric ( TTAGGG ) n sequences in eight species of Brazilian marsupials ( Didelphidae ) by FISH and the correlation with constitutive heterochromatin .
	manualset3
106061	6	402651	5	NULL	NULL	0	NULL	correlation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mapping the distribution of the interstitial telomeric ( TTAGGG ) n sequences in eight species of Brazilian marsupials ( Didelphidae ) by FISH and the correlation with constitutive heterochromatin .
	manualset3
106062	7	402651	5	NULL	NULL	0	NULL	constitutive heterochromatin	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Mapping the distribution of the interstitial telomeric ( TTAGGG ) n sequences in eight species of Brazilian marsupials ( Didelphidae ) by FISH and the correlation with constitutive heterochromatin .
	manualset3
106063	1	402652	5	NULL	NULL	0	NULL	increasing risk	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mapping the increasing risk of human alveolar echinococcosis in Limburg , The Netherlands .
	manualset3
106064	2	402652	5	NULL	NULL	0	NULL	human alveolar echinococcosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mapping the increasing risk of human alveolar echinococcosis in Limburg , The Netherlands .
	manualset3
106065	3	402652	5	NULL	NULL	0	NULL	Limburg , The Netherlands	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Mapping the increasing risk of human alveolar echinococcosis in Limburg , The Netherlands .
	manualset3
106066	1	402653	5	NULL	NULL	0	NULL	zonal organization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mapping the zonal organization of tumor perfusion and permeability in a rat glioma model by using dynamic contrast-enhanced synchrotron radiation CT .
	manualset3
106067	2	402653	5	NULL	NULL	0	NULL	tumor perfusion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mapping the zonal organization of tumor perfusion and permeability in a rat glioma model by using dynamic contrast-enhanced synchrotron radiation CT .
	manualset3
106068	3	402653	5	NULL	NULL	0	NULL	permeability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mapping the zonal organization of tumor perfusion and permeability in a rat glioma model by using dynamic contrast-enhanced synchrotron radiation CT .
	manualset3
106069	4	402653	5	NULL	NULL	0	NULL	rat glioma model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Mapping the zonal organization of tumor perfusion and permeability in a rat glioma model by using dynamic contrast-enhanced synchrotron radiation CT .
	manualset3
106070	5	402653	5	NULL	NULL	0	NULL	dynamic contrast-enhanced synchrotron radiation CT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Mapping the zonal organization of tumor perfusion and permeability in a rat glioma model by using dynamic contrast-enhanced synchrotron radiation CT .
	manualset3
106071	1	402654	5	NULL	NULL	0	NULL	Marginal attack rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Marginal attack rates and associated k-values were calculated to allow comparison of mortality factors between experimental sites .
	manualset3
106072	2	402654	5	NULL	NULL	0	NULL	k-values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Marginal attack rates and associated k-values were calculated to allow comparison of mortality factors between experimental sites .
	manualset3
106073	3	402654	5	NULL	NULL	0	NULL	comparison 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Marginal attack rates and associated k-values were calculated to allow comparison of mortality factors between experimental sites .
	manualset3
106074	4	402654	5	NULL	NULL	0	NULL	mortality factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Marginal attack rates and associated k-values were calculated to allow comparison of mortality factors between experimental sites .
	manualset3
106075	5	402654	5	NULL	NULL	0	NULL	experimental sites	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Marginal attack rates and associated k-values were calculated to allow comparison of mortality factors between experimental sites .
	manualset3
106076	1	402655	5	NULL	NULL	0	NULL	Marginalised populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Marginalised populations , including at risk young people , injecting drug users and sex workers , are vulnerable to a range of preventable health related problems , yet they often have difficulty accessing mainstream primary healthcare services .
	manualset3
106077	2	402655	5	NULL	NULL	0	NULL	risk	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Marginalised populations , including at risk young people , injecting drug users and sex workers , are vulnerable to a range of preventable health related problems , yet they often have difficulty accessing mainstream primary healthcare services .
	manualset3
106078	3	402655	5	NULL	NULL	0	NULL	young people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Marginalised populations , including at risk young people , injecting drug users and sex workers , are vulnerable to a range of preventable health related problems , yet they often have difficulty accessing mainstream primary healthcare services .
	manualset3
106079	4	402655	5	NULL	NULL	0	NULL	injecting drug users	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Marginalised populations , including at risk young people , injecting drug users and sex workers , are vulnerable to a range of preventable health related problems , yet they often have difficulty accessing mainstream primary healthcare services .
	manualset3
106080	5	402655	5	NULL	NULL	0	NULL	sex workers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Marginalised populations , including at risk young people , injecting drug users and sex workers , are vulnerable to a range of preventable health related problems , yet they often have difficulty accessing mainstream primary healthcare services .
	manualset3
106098	6	402655	5	NULL	NULL	0	NULL	range 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Marginalised populations , including at risk young people , injecting drug users and sex workers , are vulnerable to a range of preventable health related problems , yet they often have difficulty accessing mainstream primary healthcare services .
	manualset3
106099	7	402655	5	NULL	NULL	0	NULL	preventable health related problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Marginalised populations , including at risk young people , injecting drug users and sex workers , are vulnerable to a range of preventable health related problems , yet they often have difficulty accessing mainstream primary healthcare services .
	manualset3
106101	8	402655	5	NULL	NULL	0	NULL	mainstream primary healthcare services	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Marginalised populations , including at risk young people , injecting drug users and sex workers , are vulnerable to a range of preventable health related problems , yet they often have difficulty accessing mainstream primary healthcare services .
	manualset3
106106	1	402656	5	NULL	NULL	0	NULL	Maria Dbska	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Maria Dbska was a brave hero of the Warsaw Resurrection of 1944 who survived deportation to Germany to graduate from medical school in Gdask and pursue a career in pathology , for which her research on the Dbska tumor , breast cancer , sweat gland tumors , keratoacanthoma , soft tissue sarcomas , bone pathology , parachordoma , melanoma , and other entities remains salient .
	manualset3
106108	2	402656	5	NULL	NULL	0	NULL	brave hero 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Maria Dbska was a brave hero of the Warsaw Resurrection of 1944 who survived deportation to Germany to graduate from medical school in Gdask and pursue a career in pathology , for which her research on the Dbska tumor , breast cancer , sweat gland tumors , keratoacanthoma , soft tissue sarcomas , bone pathology , parachordoma , melanoma , and other entities remains salient .
	manualset3
106115	3	402656	5	NULL	NULL	0	NULL	Warsaw Resurrection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Maria Dbska was a brave hero of the Warsaw Resurrection of 1944 who survived deportation to Germany to graduate from medical school in Gdask and pursue a career in pathology , for which her research on the Dbska tumor , breast cancer , sweat gland tumors , keratoacanthoma , soft tissue sarcomas , bone pathology , parachordoma , melanoma , and other entities remains salient .
	manualset3
106117	4	402656	5	NULL	NULL	0	NULL	1944 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Maria Dbska was a brave hero of the Warsaw Resurrection of 1944 who survived deportation to Germany to graduate from medical school in Gdask and pursue a career in pathology , for which her research on the Dbska tumor , breast cancer , sweat gland tumors , keratoacanthoma , soft tissue sarcomas , bone pathology , parachordoma , melanoma , and other entities remains salient .
	manualset3
106119	5	402656	5	NULL	NULL	0	NULL	deportation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Maria Dbska was a brave hero of the Warsaw Resurrection of 1944 who survived deportation to Germany to graduate from medical school in Gdask and pursue a career in pathology , for which her research on the Dbska tumor , breast cancer , sweat gland tumors , keratoacanthoma , soft tissue sarcomas , bone pathology , parachordoma , melanoma , and other entities remains salient .
	manualset3
106120	6	402656	5	NULL	NULL	0	NULL	Germany 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Maria Dbska was a brave hero of the Warsaw Resurrection of 1944 who survived deportation to Germany to graduate from medical school in Gdask and pursue a career in pathology , for which her research on the Dbska tumor , breast cancer , sweat gland tumors , keratoacanthoma , soft tissue sarcomas , bone pathology , parachordoma , melanoma , and other entities remains salient .
	manualset3
106121	7	402656	5	NULL	NULL	0	NULL	medical school	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Maria Dbska was a brave hero of the Warsaw Resurrection of 1944 who survived deportation to Germany to graduate from medical school in Gdask and pursue a career in pathology , for which her research on the Dbska tumor , breast cancer , sweat gland tumors , keratoacanthoma , soft tissue sarcomas , bone pathology , parachordoma , melanoma , and other entities remains salient .
	manualset3
106122	8	402656	5	NULL	NULL	0	NULL	Gdask 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Maria Dbska was a brave hero of the Warsaw Resurrection of 1944 who survived deportation to Germany to graduate from medical school in Gdask and pursue a career in pathology , for which her research on the Dbska tumor , breast cancer , sweat gland tumors , keratoacanthoma , soft tissue sarcomas , bone pathology , parachordoma , melanoma , and other entities remains salient .
	manualset3
106125	9	402656	5	NULL	NULL	0	NULL	career 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Maria Dbska was a brave hero of the Warsaw Resurrection of 1944 who survived deportation to Germany to graduate from medical school in Gdask and pursue a career in pathology , for which her research on the Dbska tumor , breast cancer , sweat gland tumors , keratoacanthoma , soft tissue sarcomas , bone pathology , parachordoma , melanoma , and other entities remains salient .
	manualset3
106126	10	402656	5	NULL	NULL	0	NULL	pathology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Maria Dbska was a brave hero of the Warsaw Resurrection of 1944 who survived deportation to Germany to graduate from medical school in Gdask and pursue a career in pathology , for which her research on the Dbska tumor , breast cancer , sweat gland tumors , keratoacanthoma , soft tissue sarcomas , bone pathology , parachordoma , melanoma , and other entities remains salient .
	manualset3
106127	11	402656	5	NULL	NULL	0	NULL	research 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Maria Dbska was a brave hero of the Warsaw Resurrection of 1944 who survived deportation to Germany to graduate from medical school in Gdask and pursue a career in pathology , for which her research on the Dbska tumor , breast cancer , sweat gland tumors , keratoacanthoma , soft tissue sarcomas , bone pathology , parachordoma , melanoma , and other entities remains salient .
	manualset3
106128	12	402656	5	NULL	NULL	0	NULL	Dbska tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Maria Dbska was a brave hero of the Warsaw Resurrection of 1944 who survived deportation to Germany to graduate from medical school in Gdask and pursue a career in pathology , for which her research on the Dbska tumor , breast cancer , sweat gland tumors , keratoacanthoma , soft tissue sarcomas , bone pathology , parachordoma , melanoma , and other entities remains salient .
	manualset3
106129	13	402656	5	NULL	NULL	0	NULL	breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Maria Dbska was a brave hero of the Warsaw Resurrection of 1944 who survived deportation to Germany to graduate from medical school in Gdask and pursue a career in pathology , for which her research on the Dbska tumor , breast cancer , sweat gland tumors , keratoacanthoma , soft tissue sarcomas , bone pathology , parachordoma , melanoma , and other entities remains salient .
	manualset3
106130	14	402656	5	NULL	NULL	0	NULL	sweat gland tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Maria Dbska was a brave hero of the Warsaw Resurrection of 1944 who survived deportation to Germany to graduate from medical school in Gdask and pursue a career in pathology , for which her research on the Dbska tumor , breast cancer , sweat gland tumors , keratoacanthoma , soft tissue sarcomas , bone pathology , parachordoma , melanoma , and other entities remains salient .
	manualset3
106131	15	402656	5	NULL	NULL	0	NULL	keratoacanthoma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Maria Dbska was a brave hero of the Warsaw Resurrection of 1944 who survived deportation to Germany to graduate from medical school in Gdask and pursue a career in pathology , for which her research on the Dbska tumor , breast cancer , sweat gland tumors , keratoacanthoma , soft tissue sarcomas , bone pathology , parachordoma , melanoma , and other entities remains salient .
	manualset3
106132	16	402656	5	NULL	NULL	0	NULL	soft tissue sarcomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Maria Dbska was a brave hero of the Warsaw Resurrection of 1944 who survived deportation to Germany to graduate from medical school in Gdask and pursue a career in pathology , for which her research on the Dbska tumor , breast cancer , sweat gland tumors , keratoacanthoma , soft tissue sarcomas , bone pathology , parachordoma , melanoma , and other entities remains salient .
	manualset3
106133	17	402656	5	NULL	NULL	0	NULL	bone pathology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Maria Dbska was a brave hero of the Warsaw Resurrection of 1944 who survived deportation to Germany to graduate from medical school in Gdask and pursue a career in pathology , for which her research on the Dbska tumor , breast cancer , sweat gland tumors , keratoacanthoma , soft tissue sarcomas , bone pathology , parachordoma , melanoma , and other entities remains salient .
	manualset3
106136	18	402656	5	NULL	NULL	0	NULL	parachordoma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Maria Dbska was a brave hero of the Warsaw Resurrection of 1944 who survived deportation to Germany to graduate from medical school in Gdask and pursue a career in pathology , for which her research on the Dbska tumor , breast cancer , sweat gland tumors , keratoacanthoma , soft tissue sarcomas , bone pathology , parachordoma , melanoma , and other entities remains salient .
	manualset3
106138	19	402656	5	NULL	NULL	0	NULL	melanoma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Maria Dbska was a brave hero of the Warsaw Resurrection of 1944 who survived deportation to Germany to graduate from medical school in Gdask and pursue a career in pathology , for which her research on the Dbska tumor , breast cancer , sweat gland tumors , keratoacanthoma , soft tissue sarcomas , bone pathology , parachordoma , melanoma , and other entities remains salient .
	manualset3
106140	20	402656	5	NULL	NULL	0	NULL	other entities	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Maria Dbska was a brave hero of the Warsaw Resurrection of 1944 who survived deportation to Germany to graduate from medical school in Gdask and pursue a career in pathology , for which her research on the Dbska tumor , breast cancer , sweat gland tumors , keratoacanthoma , soft tissue sarcomas , bone pathology , parachordoma , melanoma , and other entities remains salient .
	manualset3
106143	1	402657	5	NULL	NULL	0	NULL	Marked elevation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked elevation of urinary alpha G-K was also noted following oral treatment of adult male rats with 2 , 2 , 4-trimethylpentane ( TMP ) , 1 , 4-dichlorobenzene ( DCB ) , decalin and isophorone ( ISP ) by gavage ( 1.5 mmol/kg/day ) for 7 consecutive days , again in association with increased concentrations of renal alpha G-K and hyaline droplet accumulation in renal PCT epithelial cells .
	manualset3
106149	2	402657	5	NULL	NULL	0	NULL	urinary alpha G-K	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked elevation of urinary alpha G-K was also noted following oral treatment of adult male rats with 2 , 2 , 4-trimethylpentane ( TMP ) , 1 , 4-dichlorobenzene ( DCB ) , decalin and isophorone ( ISP ) by gavage ( 1.5 mmol/kg/day ) for 7 consecutive days , again in association with increased concentrations of renal alpha G-K and hyaline droplet accumulation in renal PCT epithelial cells .
	manualset3
106151	3	402657	5	NULL	NULL	0	NULL	oral treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked elevation of urinary alpha G-K was also noted following oral treatment of adult male rats with 2 , 2 , 4-trimethylpentane ( TMP ) , 1 , 4-dichlorobenzene ( DCB ) , decalin and isophorone ( ISP ) by gavage ( 1.5 mmol/kg/day ) for 7 consecutive days , again in association with increased concentrations of renal alpha G-K and hyaline droplet accumulation in renal PCT epithelial cells .
	manualset3
106152	4	402657	5	NULL	NULL	0	NULL	adult male rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked elevation of urinary alpha G-K was also noted following oral treatment of adult male rats with 2 , 2 , 4-trimethylpentane ( TMP ) , 1 , 4-dichlorobenzene ( DCB ) , decalin and isophorone ( ISP ) by gavage ( 1.5 mmol/kg/day ) for 7 consecutive days , again in association with increased concentrations of renal alpha G-K and hyaline droplet accumulation in renal PCT epithelial cells .
	manualset3
106155	5	402657	5	NULL	NULL	0	NULL	2 , 2 , 4-trimethylpentane ( TMP )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked elevation of urinary alpha G-K was also noted following oral treatment of adult male rats with 2 , 2 , 4-trimethylpentane ( TMP ) , 1 , 4-dichlorobenzene ( DCB ) , decalin and isophorone ( ISP ) by gavage ( 1.5 mmol/kg/day ) for 7 consecutive days , again in association with increased concentrations of renal alpha G-K and hyaline droplet accumulation in renal PCT epithelial cells .
	manualset3
106163	6	402657	5	NULL	NULL	0	NULL	1 , 4-dichlorobenzene ( DCB )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked elevation of urinary alpha G-K was also noted following oral treatment of adult male rats with 2 , 2 , 4-trimethylpentane ( TMP ) , 1 , 4-dichlorobenzene ( DCB ) , decalin and isophorone ( ISP ) by gavage ( 1.5 mmol/kg/day ) for 7 consecutive days , again in association with increased concentrations of renal alpha G-K and hyaline droplet accumulation in renal PCT epithelial cells .
	manualset3
106165	7	402657	5	NULL	NULL	0	NULL	decalin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked elevation of urinary alpha G-K was also noted following oral treatment of adult male rats with 2 , 2 , 4-trimethylpentane ( TMP ) , 1 , 4-dichlorobenzene ( DCB ) , decalin and isophorone ( ISP ) by gavage ( 1.5 mmol/kg/day ) for 7 consecutive days , again in association with increased concentrations of renal alpha G-K and hyaline droplet accumulation in renal PCT epithelial cells .
	manualset3
106166	8	402657	5	NULL	NULL	0	NULL	isophorone ( ISP ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked elevation of urinary alpha G-K was also noted following oral treatment of adult male rats with 2 , 2 , 4-trimethylpentane ( TMP ) , 1 , 4-dichlorobenzene ( DCB ) , decalin and isophorone ( ISP ) by gavage ( 1.5 mmol/kg/day ) for 7 consecutive days , again in association with increased concentrations of renal alpha G-K and hyaline droplet accumulation in renal PCT epithelial cells .
	manualset3
106167	9	402657	5	NULL	NULL	0	NULL	gavage 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked elevation of urinary alpha G-K was also noted following oral treatment of adult male rats with 2 , 2 , 4-trimethylpentane ( TMP ) , 1 , 4-dichlorobenzene ( DCB ) , decalin and isophorone ( ISP ) by gavage ( 1.5 mmol/kg/day ) for 7 consecutive days , again in association with increased concentrations of renal alpha G-K and hyaline droplet accumulation in renal PCT epithelial cells .
	manualset3
106168	10	402657	5	NULL	NULL	0	NULL	1.5 mmol/kg/day 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked elevation of urinary alpha G-K was also noted following oral treatment of adult male rats with 2 , 2 , 4-trimethylpentane ( TMP ) , 1 , 4-dichlorobenzene ( DCB ) , decalin and isophorone ( ISP ) by gavage ( 1.5 mmol/kg/day ) for 7 consecutive days , again in association with increased concentrations of renal alpha G-K and hyaline droplet accumulation in renal PCT epithelial cells .
	manualset3
106169	11	402657	5	NULL	NULL	0	NULL	7 consecutive days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked elevation of urinary alpha G-K was also noted following oral treatment of adult male rats with 2 , 2 , 4-trimethylpentane ( TMP ) , 1 , 4-dichlorobenzene ( DCB ) , decalin and isophorone ( ISP ) by gavage ( 1.5 mmol/kg/day ) for 7 consecutive days , again in association with increased concentrations of renal alpha G-K and hyaline droplet accumulation in renal PCT epithelial cells .
	manualset3
106170	12	402657	5	NULL	NULL	0	NULL	association 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked elevation of urinary alpha G-K was also noted following oral treatment of adult male rats with 2 , 2 , 4-trimethylpentane ( TMP ) , 1 , 4-dichlorobenzene ( DCB ) , decalin and isophorone ( ISP ) by gavage ( 1.5 mmol/kg/day ) for 7 consecutive days , again in association with increased concentrations of renal alpha G-K and hyaline droplet accumulation in renal PCT epithelial cells .
	manualset3
106171	13	402657	5	NULL	NULL	0	NULL	increased concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked elevation of urinary alpha G-K was also noted following oral treatment of adult male rats with 2 , 2 , 4-trimethylpentane ( TMP ) , 1 , 4-dichlorobenzene ( DCB ) , decalin and isophorone ( ISP ) by gavage ( 1.5 mmol/kg/day ) for 7 consecutive days , again in association with increased concentrations of renal alpha G-K and hyaline droplet accumulation in renal PCT epithelial cells .
	manualset3
106172	14	402657	5	NULL	NULL	0	NULL	renal alpha G-K	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked elevation of urinary alpha G-K was also noted following oral treatment of adult male rats with 2 , 2 , 4-trimethylpentane ( TMP ) , 1 , 4-dichlorobenzene ( DCB ) , decalin and isophorone ( ISP ) by gavage ( 1.5 mmol/kg/day ) for 7 consecutive days , again in association with increased concentrations of renal alpha G-K and hyaline droplet accumulation in renal PCT epithelial cells .
	manualset3
106173	15	402657	5	NULL	NULL	0	NULL	hyaline droplet accumulation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked elevation of urinary alpha G-K was also noted following oral treatment of adult male rats with 2 , 2 , 4-trimethylpentane ( TMP ) , 1 , 4-dichlorobenzene ( DCB ) , decalin and isophorone ( ISP ) by gavage ( 1.5 mmol/kg/day ) for 7 consecutive days , again in association with increased concentrations of renal alpha G-K and hyaline droplet accumulation in renal PCT epithelial cells .
	manualset3
106174	16	402657	5	NULL	NULL	0	NULL	renal PCT epithelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked elevation of urinary alpha G-K was also noted following oral treatment of adult male rats with 2 , 2 , 4-trimethylpentane ( TMP ) , 1 , 4-dichlorobenzene ( DCB ) , decalin and isophorone ( ISP ) by gavage ( 1.5 mmol/kg/day ) for 7 consecutive days , again in association with increased concentrations of renal alpha G-K and hyaline droplet accumulation in renal PCT epithelial cells .
	manualset3
106175	1	402658	5	NULL	NULL	0	NULL	RAW264 .7 macrophage cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A RAW264 .7 macrophage cell line was stimulated with four strains of KLAB and two strains of bifidobacteria , and then the production of nitric oxide ( NO ) and cytokines -- tumor necrosis factor-alpha ( TNF-alpha ) and interleukin-6 ( IL-6 ) -- was determined .
	manualset3
106176	2	402658	5	NULL	NULL	0	NULL	four strains of KLAB	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A RAW264 .7 macrophage cell line was stimulated with four strains of KLAB and two strains of bifidobacteria , and then the production of nitric oxide ( NO ) and cytokines -- tumor necrosis factor-alpha ( TNF-alpha ) and interleukin-6 ( IL-6 ) -- was determined .
	manualset3
106177	3	402658	5	NULL	NULL	0	NULL	 two strains of bifidobacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A RAW264 .7 macrophage cell line was stimulated with four strains of KLAB and two strains of bifidobacteria , and then the production of nitric oxide ( NO ) and cytokines -- tumor necrosis factor-alpha ( TNF-alpha ) and interleukin-6 ( IL-6 ) -- was determined .
	manualset3
106178	4	402658	5	NULL	NULL	0	NULL	production 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A RAW264 .7 macrophage cell line was stimulated with four strains of KLAB and two strains of bifidobacteria , and then the production of nitric oxide ( NO ) and cytokines -- tumor necrosis factor-alpha ( TNF-alpha ) and interleukin-6 ( IL-6 ) -- was determined .
	manualset3
106179	5	402658	5	NULL	NULL	0	NULL	nitric oxide ( NO )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A RAW264 .7 macrophage cell line was stimulated with four strains of KLAB and two strains of bifidobacteria , and then the production of nitric oxide ( NO ) and cytokines -- tumor necrosis factor-alpha ( TNF-alpha ) and interleukin-6 ( IL-6 ) -- was determined .
	manualset3
106180	6	402658	5	NULL	NULL	0	NULL	cytokines 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A RAW264 .7 macrophage cell line was stimulated with four strains of KLAB and two strains of bifidobacteria , and then the production of nitric oxide ( NO ) and cytokines -- tumor necrosis factor-alpha ( TNF-alpha ) and interleukin-6 ( IL-6 ) -- was determined .
	manualset3
106181	7	402658	5	NULL	NULL	0	NULL	tumor necrosis factor-alpha ( TNF-alpha )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A RAW264 .7 macrophage cell line was stimulated with four strains of KLAB and two strains of bifidobacteria , and then the production of nitric oxide ( NO ) and cytokines -- tumor necrosis factor-alpha ( TNF-alpha ) and interleukin-6 ( IL-6 ) -- was determined .
	manualset3
106182	8	402658	5	NULL	NULL	0	NULL	interleukin-6 ( IL-6 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A RAW264 .7 macrophage cell line was stimulated with four strains of KLAB and two strains of bifidobacteria , and then the production of nitric oxide ( NO ) and cytokines -- tumor necrosis factor-alpha ( TNF-alpha ) and interleukin-6 ( IL-6 ) -- was determined .
	manualset3
106208	1	402659	5	NULL	NULL	0	NULL	Type III acromions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked increase in contact with Type III acromions supports the role of anterior acromioplasty when clinically indicated , usually in older patients with primary impingement .
	manualset3
106211	2	402659	5	NULL	NULL	0	NULL	anterior acromioplasty	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked increase in contact with Type III acromions supports the role of anterior acromioplasty when clinically indicated , usually in older patients with primary impingement .
	manualset3
106215	3	402659	5	NULL	NULL	0	NULL	older patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked increase in contact with Type III acromions supports the role of anterior acromioplasty when clinically indicated , usually in older patients with primary impingement .
	manualset3
106220	4	402659	5	NULL	NULL	0	NULL	primary impingement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked increase in contact with Type III acromions supports the role of anterior acromioplasty when clinically indicated , usually in older patients with primary impingement .
	manualset3
106223	1	402660	5	NULL	NULL	0	NULL	toxicity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked toxicity was observed following incubation of benoxaprofen with isolated hepatocytes from either untreated , phenobarbitone ( PB ) or 3-methylcholanthrene ( 3-MC ) pretreated male rats .
	manualset3
106224	2	402660	5	NULL	NULL	0	NULL	incubation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked toxicity was observed following incubation of benoxaprofen with isolated hepatocytes from either untreated , phenobarbitone ( PB ) or 3-methylcholanthrene ( 3-MC ) pretreated male rats .
	manualset3
106225	3	402660	5	NULL	NULL	0	NULL	benoxaprofen 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked toxicity was observed following incubation of benoxaprofen with isolated hepatocytes from either untreated , phenobarbitone ( PB ) or 3-methylcholanthrene ( 3-MC ) pretreated male rats .
	manualset3
106226	4	402660	5	NULL	NULL	0	NULL	isolated hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked toxicity was observed following incubation of benoxaprofen with isolated hepatocytes from either untreated , phenobarbitone ( PB ) or 3-methylcholanthrene ( 3-MC ) pretreated male rats .
	manualset3
106227	5	402660	5	NULL	NULL	0	NULL	untreated , phenobarbitone ( PB )  male rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked toxicity was observed following incubation of benoxaprofen with isolated hepatocytes from either untreated , phenobarbitone ( PB ) or 3-methylcholanthrene ( 3-MC ) pretreated male rats .
	manualset3
106228	6	402660	5	NULL	NULL	0	NULL	3-methylcholanthrene ( 3-MC ) pretreated male rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked toxicity was observed following incubation of benoxaprofen with isolated hepatocytes from either untreated , phenobarbitone ( PB ) or 3-methylcholanthrene ( 3-MC ) pretreated male rats .
	manualset3
106467	1	402661	5	NULL	NULL	0	NULL	Markers 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Markers derived from occupational exposure assessment , questionnaires , clinical data , and noninvasive tests such as functional tests or measures of serum antibodies are used to develop prediction models for the likelihood of OA and OR development .
	manualset3
106468	2	402661	5	NULL	NULL	0	NULL	occupational exposure assessment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Markers derived from occupational exposure assessment , questionnaires , clinical data , and noninvasive tests such as functional tests or measures of serum antibodies are used to develop prediction models for the likelihood of OA and OR development .
	manualset3
106469	3	402661	5	NULL	NULL	0	NULL	questionnaires 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Markers derived from occupational exposure assessment , questionnaires , clinical data , and noninvasive tests such as functional tests or measures of serum antibodies are used to develop prediction models for the likelihood of OA and OR development .
	manualset3
106470	4	402661	5	NULL	NULL	0	NULL	clinical data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Markers derived from occupational exposure assessment , questionnaires , clinical data , and noninvasive tests such as functional tests or measures of serum antibodies are used to develop prediction models for the likelihood of OA and OR development .
	manualset3
106471	5	402661	5	NULL	NULL	0	NULL	noninvasive tests	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Markers derived from occupational exposure assessment , questionnaires , clinical data , and noninvasive tests such as functional tests or measures of serum antibodies are used to develop prediction models for the likelihood of OA and OR development .
	manualset3
106472	6	402661	5	NULL	NULL	0	NULL	functional tests	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Markers derived from occupational exposure assessment , questionnaires , clinical data , and noninvasive tests such as functional tests or measures of serum antibodies are used to develop prediction models for the likelihood of OA and OR development .
	manualset3
106473	7	402661	5	NULL	NULL	0	NULL	measures 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Markers derived from occupational exposure assessment , questionnaires , clinical data , and noninvasive tests such as functional tests or measures of serum antibodies are used to develop prediction models for the likelihood of OA and OR development .
	manualset3
106474	8	402661	5	NULL	NULL	0	NULL	serum antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Markers derived from occupational exposure assessment , questionnaires , clinical data , and noninvasive tests such as functional tests or measures of serum antibodies are used to develop prediction models for the likelihood of OA and OR development .
	manualset3
106475	9	402661	5	NULL	NULL	0	NULL	prediction models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Markers derived from occupational exposure assessment , questionnaires , clinical data , and noninvasive tests such as functional tests or measures of serum antibodies are used to develop prediction models for the likelihood of OA and OR development .
	manualset3
106476	10	402661	5	NULL	NULL	0	NULL	OA development	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Markers derived from occupational exposure assessment , questionnaires , clinical data , and noninvasive tests such as functional tests or measures of serum antibodies are used to develop prediction models for the likelihood of OA and OR development .
	manualset3
106477	11	402661	5	NULL	NULL	0	NULL	OR development	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Markers derived from occupational exposure assessment , questionnaires , clinical data , and noninvasive tests such as functional tests or measures of serum antibodies are used to develop prediction models for the likelihood of OA and OR development .
	manualset3
106478	1	402662	5	NULL	NULL	0	NULL	Markers 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Markers of increased angiogenesis and their correlation with biological parameters identifying high-risk patients in early B-cell chronic lymphocytic leukemia .
	manualset3
106479	2	402662	5	NULL	NULL	0	NULL	angiogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Markers of increased angiogenesis and their correlation with biological parameters identifying high-risk patients in early B-cell chronic lymphocytic leukemia .
	manualset3
106480	3	402662	5	NULL	NULL	0	NULL	correlation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Markers of increased angiogenesis and their correlation with biological parameters identifying high-risk patients in early B-cell chronic lymphocytic leukemia .
	manualset3
106481	4	402662	5	NULL	NULL	0	NULL	biological parameters	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Markers of increased angiogenesis and their correlation with biological parameters identifying high-risk patients in early B-cell chronic lymphocytic leukemia .
	manualset3
106482	5	402662	5	NULL	NULL	0	NULL	high-risk patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Markers of increased angiogenesis and their correlation with biological parameters identifying high-risk patients in early B-cell chronic lymphocytic leukemia .
	manualset3
106483	6	402662	5	NULL	NULL	0	NULL	early B-cell chronic lymphocytic leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Markers of increased angiogenesis and their correlation with biological parameters identifying high-risk patients in early B-cell chronic lymphocytic leukemia .
	manualset3
106484	1	402663	5	NULL	NULL	0	NULL	Market accountability	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Market accountability requires plans to inform purchasers and consumers about performance and options , in theory legitimizing limits to care through consumer choice .
	manualset3
106485	2	402663	5	NULL	NULL	0	NULL	plans 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Market accountability requires plans to inform purchasers and consumers about performance and options , in theory legitimizing limits to care through consumer choice .
	manualset3
106486	3	402663	5	NULL	NULL	0	NULL	purchasers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Market accountability requires plans to inform purchasers and consumers about performance and options , in theory legitimizing limits to care through consumer choice .
	manualset3
106487	4	402663	5	NULL	NULL	0	NULL	consumers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Market accountability requires plans to inform purchasers and consumers about performance and options , in theory legitimizing limits to care through consumer choice .
	manualset3
106488	5	402663	5	NULL	NULL	0	NULL	performance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Market accountability requires plans to inform purchasers and consumers about performance and options , in theory legitimizing limits to care through consumer choice .
	manualset3
106489	6	402663	5	NULL	NULL	0	NULL	options 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Market accountability requires plans to inform purchasers and consumers about performance and options , in theory legitimizing limits to care through consumer choice .
	manualset3
106490	7	402663	5	NULL	NULL	0	NULL	theory 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Market accountability requires plans to inform purchasers and consumers about performance and options , in theory legitimizing limits to care through consumer choice .
	manualset3
106491	8	402663	5	NULL	NULL	0	NULL	limits 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Market accountability requires plans to inform purchasers and consumers about performance and options , in theory legitimizing limits to care through consumer choice .
	manualset3
106492	9	402663	5	NULL	NULL	0	NULL	care 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Market accountability requires plans to inform purchasers and consumers about performance and options , in theory legitimizing limits to care through consumer choice .
	manualset3
106493	10	402663	5	NULL	NULL	0	NULL	consumer choice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Market accountability requires plans to inform purchasers and consumers about performance and options , in theory legitimizing limits to care through consumer choice .
	manualset3
106494	1	402664	5	NULL	NULL	0	NULL	Market research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Market research should be conducted in order to ascertain consumer likes and dislikes .
	manualset3
106495	2	402664	5	NULL	NULL	NULL	NULL	consumer likes	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Market research should be conducted in order to ascertain consumer likes and dislikes .
	manualset3
106496	3	402664	5	NULL	NULL	0	NULL	consumer dislikes	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Market research should be conducted in order to ascertain consumer likes and dislikes .
	manualset3
106497	1	402665	5	NULL	NULL	0	NULL	SNP	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A SNP based linkage map of the turkey genome reveals multiple intrachromosomal rearrangements between the turkey and chicken genomes .
	manualset3
106498	2	402665	5	NULL	NULL	0	NULL	linkage map	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A SNP based linkage map of the turkey genome reveals multiple intrachromosomal rearrangements between the turkey and chicken genomes .
	manualset3
106499	3	402665	5	NULL	NULL	0	NULL	turkey genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A SNP based linkage map of the turkey genome reveals multiple intrachromosomal rearrangements between the turkey and chicken genomes .
	manualset3
106500	4	402665	5	NULL	NULL	0	NULL	multiple intrachromosomal rearrangements	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A SNP based linkage map of the turkey genome reveals multiple intrachromosomal rearrangements between the turkey and chicken genomes .
	manualset3
106501	5	402665	5	NULL	NULL	0	NULL	turkey genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A SNP based linkage map of the turkey genome reveals multiple intrachromosomal rearrangements between the turkey and chicken genomes .
	manualset3
106502	6	402665	5	NULL	NULL	0	NULL	chicken genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A SNP based linkage map of the turkey genome reveals multiple intrachromosomal rearrangements between the turkey and chicken genomes .
	manualset3
106503	1	402666	5	NULL	NULL	0	NULL	Marrow cell uptake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Marrow cell uptake by megakaryocytes and naked megakaryocyte nuclei in routine bone marrow examination .
	manualset3
106504	2	402666	5	NULL	NULL	0	NULL	megakaryocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Marrow cell uptake by megakaryocytes and naked megakaryocyte nuclei in routine bone marrow examination .
	manualset3
106505	3	402666	5	NULL	NULL	0	NULL	naked megakaryocyte nuclei	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Marrow cell uptake by megakaryocytes and naked megakaryocyte nuclei in routine bone marrow examination .
	manualset3
106506	4	402666	5	NULL	NULL	0	NULL	routine bone marrow examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Marrow cell uptake by megakaryocytes and naked megakaryocyte nuclei in routine bone marrow examination .
	manualset3
106507	1	402667	5	NULL	NULL	NULL	NULL	Marrubiin concentration 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Marrubiin , phlomeoic acid , RA , and RB concentration dependently ( 3.0-10 g/mL ) shifted the Ca ( + + ) curves to the right obtained in Ca ( + + ) - free medium .
	manualset3
106508	2	402667	5	NULL	NULL	NULL	NULL	phlomeoic acid concentration 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Marrubiin , phlomeoic acid , RA , and RB concentration dependently ( 3.0-10 g/mL ) shifted the Ca ( + + ) curves to the right obtained in Ca ( + + ) - free medium .
	manualset3
106509	3	402667	5	NULL	NULL	0	NULL	RA concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Marrubiin , phlomeoic acid , RA , and RB concentration dependently ( 3.0-10 g/mL ) shifted the Ca ( + + ) curves to the right obtained in Ca ( + + ) - free medium .
	manualset3
106510	4	402667	5	NULL	NULL	0	NULL	RB concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Marrubiin , phlomeoic acid , RA , and RB concentration dependently ( 3.0-10 g/mL ) shifted the Ca ( + + ) curves to the right obtained in Ca ( + + ) - free medium .
	manualset3
106511	5	402667	5	NULL	NULL	0	NULL	3.0-10 g/mL 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Marrubiin , phlomeoic acid , RA , and RB concentration dependently ( 3.0-10 g/mL ) shifted the Ca ( + + ) curves to the right obtained in Ca ( + + ) - free medium .
	manualset3
106512	6	402667	5	NULL	NULL	0	NULL	Ca ( + + ) curves	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Marrubiin , phlomeoic acid , RA , and RB concentration dependently ( 3.0-10 g/mL ) shifted the Ca ( + + ) curves to the right obtained in Ca ( + + ) - free medium .
	manualset3
106513	7	402667	5	NULL	NULL	0	NULL	Ca ( + + ) - free medium 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Marrubiin , phlomeoic acid , RA , and RB concentration dependently ( 3.0-10 g/mL ) shifted the Ca ( + + ) curves to the right obtained in Ca ( + + ) - free medium .
	manualset3
106514	1	402668	5	NULL	NULL	0	NULL	Mass gatherings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mass gatherings are an increasingly common feature of modern society .
	manualset3
106515	2	402668	5	NULL	NULL	0	NULL	modern society	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mass gatherings are an increasingly common feature of modern society .
	manualset3
106516	1	402669	5	NULL	NULL	0	NULL	Mass spectrometric analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mass spectrometric analysis of cross-linked homo - and heterotetramers reveals species of distinct molecular mass for HGPRT-I , HGPRT-II , and HGPRT-I .
	manualset3
106517	1	402669	5	NULL	NULL	0	NULL	Mass spectrometric analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mass spectrometric analysis of cross-linked homo - and heterotetramers reveals species of distinct molecular mass for HGPRT-I , HGPRT-II , and HGPRT-I .
	manualset3
106518	2	402669	5	NULL	NULL	0	NULL	cross-linked homo - and heterotetramers	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mass spectrometric analysis of cross-linked homo - and heterotetramers reveals species of distinct molecular mass for HGPRT-I , HGPRT-II , and HGPRT-I .
	manualset3
106519	3	402669	5	NULL	NULL	0	NULL	species 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mass spectrometric analysis of cross-linked homo - and heterotetramers reveals species of distinct molecular mass for HGPRT-I , HGPRT-II , and HGPRT-I .
	manualset3
106520	4	402669	5	NULL	NULL	0	NULL	distinct molecular mass	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mass spectrometric analysis of cross-linked homo - and heterotetramers reveals species of distinct molecular mass for HGPRT-I , HGPRT-II , and HGPRT-I .
	manualset3
106521	5	402669	5	NULL	NULL	0	NULL	HGPRT-I	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mass spectrometric analysis of cross-linked homo - and heterotetramers reveals species of distinct molecular mass for HGPRT-I , HGPRT-II , and HGPRT-I .
	manualset3
106522	6	402669	5	NULL	NULL	0	NULL	HGPRT-II	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mass spectrometric analysis of cross-linked homo - and heterotetramers reveals species of distinct molecular mass for HGPRT-I , HGPRT-II , and HGPRT-I .
	manualset3
106523	7	402669	5	NULL	NULL	0	NULL	HGPRT-I	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mass spectrometric analysis of cross-linked homo - and heterotetramers reveals species of distinct molecular mass for HGPRT-I , HGPRT-II , and HGPRT-I .
	manualset3
106524	1	402670	5	NULL	NULL	0	NULL	Mass spectrometry analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mass spectrometry analysis of oxidized phosphatidylcholine and phosphatidylethanolamine .
	manualset3
106525	2	402670	5	NULL	NULL	0	NULL	oxidized phosphatidylcholine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Mass spectrometry analysis of oxidized phosphatidylcholine and phosphatidylethanolamine .
	manualset3
106526	3	402670	5	NULL	NULL	0	NULL	phosphatidylethanolamine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Mass spectrometry analysis of oxidized phosphatidylcholine and phosphatidylethanolamine .
	manualset3
106527	1	402671	5	NULL	NULL	0	NULL	SPARC 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106528	2	402671	5	NULL	NULL	0	NULL	significant positive correlation	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106529	3	402671	5	NULL	NULL	0	NULL	platelet count 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106530	4	402671	5	NULL	NULL	0	NULL	 r = 0.72	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106531	5	402671	5	NULL	NULL	0	NULL	p = 0.000000	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106532	6	402671	5	NULL	NULL	0	NULL	n = 42	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106533	7	402671	5	NULL	NULL	0	NULL	hemoglobin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106534	8	402671	5	NULL	NULL	0	NULL	r = 0.52	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106535	9	402671	5	NULL	NULL	0	NULL	p = 0.00037	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106536	10	402671	5	NULL	NULL	0	NULL	n = 42	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106537	11	402671	5	NULL	NULL	0	NULL	IgG level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106538	12	402671	5	NULL	NULL	0	NULL	r = 0.43	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106539	13	402671	5	NULL	NULL	0	NULL	p = 0.0085 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106540	14	402671	5	NULL	NULL	0	NULL	n = 42	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106541	15	402671	5	NULL	NULL	0	NULL	negative correlation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106542	16	402671	5	NULL	NULL	0	NULL	beta ( 2 ) - microglobulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106543	17	402671	5	NULL	NULL	0	NULL	 r = -0.46 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106544	18	402671	5	NULL	NULL	0	NULL	 p = 0.0023	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106545	19	402671	5	NULL	NULL	0	NULL	n = 42	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106546	20	402671	5	NULL	NULL	0	NULL	aspartate aminotransferase ( AST )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106547	21	402671	5	NULL	NULL	0	NULL	r = -0.42 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106548	22	402671	5	NULL	NULL	0	NULL	p = 0.0061 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106549	23	402671	5	NULL	NULL	0	NULL	n = 41	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106550	24	402671	5	NULL	NULL	0	NULL	interleukin ( IL ) -6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106551	25	402671	5	NULL	NULL	0	NULL	r = -0.41	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106552	26	402671	5	NULL	NULL	0	NULL	p = 0.008	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106553	27	402671	5	NULL	NULL	0	NULL	n = 42	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106554	28	402671	5	NULL	NULL	0	NULL	lactate dehydrogenase ( LDH )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106555	29	402671	5	NULL	NULL	0	NULL	r = -0.36 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106556	30	402671	5	NULL	NULL	0	NULL	p = 0.02 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106557	31	402671	5	NULL	NULL	0	NULL	n = 41	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106558	32	402671	5	NULL	NULL	0	NULL	percentage 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106559	33	402671	5	NULL	NULL	0	NULL	plasma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106560	34	402671	5	NULL	NULL	0	NULL	bone marrow aspirate	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106561	35	402671	5	NULL	NULL	0	NULL	r = -0.34	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106562	36	402671	5	NULL	NULL	0	NULL	p = 0.029	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106563	37	402671	5	NULL	NULL	0	NULL	n = 42	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A SPARC showed a significant positive correlation with platelet count ( r = 0.72 , p = 0.000000 , n = 42 ) , hemoglobin ( r = 0.52 , p = 0.00037 , n = 42 ) , and IgG level ( r = 0.43 , p = 0.0085 , n = 42 ) and negative correlation with beta ( 2 ) - microglobulin ( r = -0.46 , p = 0.0023 , n = 42 ) , aspartate aminotransferase ( AST ) ( r = -0.42 , p = 0.0061 , n = 41 ) , interleukin ( IL ) -6 ( r = -0.41 , p = 0.008 , n = 42 ) , lactate dehydrogenase ( LDH ) ( r = -0.36 , p = 0.02 , n = 41 ) , and percentage of plasma cells in bone marrow aspirate ( r = -0.34 , p = 0.029 , n = 42 ) .
	manualset3
106564	1	402672	5	NULL	NULL	0	NULL	Mast cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mast cells first appear in the pia on embryonic day ( E ) 13-14 in ovo , then along blood vessels extending from the pia into the telencephalon on posthatch day 4-5 , and in the medial habenula at week 3 .
	manualset3
106565	2	402672	5	NULL	NULL	0	NULL	pia	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mast cells first appear in the pia on embryonic day ( E ) 13-14 in ovo , then along blood vessels extending from the pia into the telencephalon on posthatch day 4-5 , and in the medial habenula at week 3 .
	manualset3
106566	3	402672	5	NULL	NULL	0	NULL	embryonic day ( E ) 13-14	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Mast cells first appear in the pia on embryonic day ( E ) 13-14 in ovo , then along blood vessels extending from the pia into the telencephalon on posthatch day 4-5 , and in the medial habenula at week 3 .
	manualset3
106567	4	402672	5	NULL	NULL	0	NULL	blood vessels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mast cells first appear in the pia on embryonic day ( E ) 13-14 in ovo , then along blood vessels extending from the pia into the telencephalon on posthatch day 4-5 , and in the medial habenula at week 3 .
	manualset3
106568	5	402672	5	NULL	NULL	0	NULL	pia 	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mast cells first appear in the pia on embryonic day ( E ) 13-14 in ovo , then along blood vessels extending from the pia into the telencephalon on posthatch day 4-5 , and in the medial habenula at week 3 .
	manualset3
106569	6	402672	5	NULL	NULL	0	NULL	telencephalon 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mast cells first appear in the pia on embryonic day ( E ) 13-14 in ovo , then along blood vessels extending from the pia into the telencephalon on posthatch day 4-5 , and in the medial habenula at week 3 .
	manualset3
106570	7	402672	5	NULL	NULL	0	NULL	posthatch day 4-5	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Mast cells first appear in the pia on embryonic day ( E ) 13-14 in ovo , then along blood vessels extending from the pia into the telencephalon on posthatch day 4-5 , and in the medial habenula at week 3 .
	manualset3
106571	8	402672	5	NULL	NULL	0	NULL	medial habenula	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mast cells first appear in the pia on embryonic day ( E ) 13-14 in ovo , then along blood vessels extending from the pia into the telencephalon on posthatch day 4-5 , and in the medial habenula at week 3 .
	manualset3
106572	9	402672	5	NULL	NULL	0	NULL	week 3	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Mast cells first appear in the pia on embryonic day ( E ) 13-14 in ovo , then along blood vessels extending from the pia into the telencephalon on posthatch day 4-5 , and in the medial habenula at week 3 .
	manualset3
106573	1	402673	5	NULL	NULL	0	NULL	Mast cell colonies	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mast cell colonies were obtained when lymph node cells of horse serum-immunized Balb/c mice were cultured in a horse serum-containing medium on embryonic fibroblast monolayer .
	manualset3
106574	2	402673	5	NULL	NULL	0	NULL	lymph node cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mast cell colonies were obtained when lymph node cells of horse serum-immunized Balb/c mice were cultured in a horse serum-containing medium on embryonic fibroblast monolayer .
	manualset3
106575	3	402673	5	NULL	NULL	0	NULL	horse serum-immunized Balb/c mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mast cell colonies were obtained when lymph node cells of horse serum-immunized Balb/c mice were cultured in a horse serum-containing medium on embryonic fibroblast monolayer .
	manualset3
106576	4	402673	5	NULL	NULL	0	NULL	horse serum-containing medium	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Mast cell colonies were obtained when lymph node cells of horse serum-immunized Balb/c mice were cultured in a horse serum-containing medium on embryonic fibroblast monolayer .
	manualset3
106577	5	402673	5	NULL	NULL	0	NULL	embryonic fibroblast monolayer	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Mast cell colonies were obtained when lymph node cells of horse serum-immunized Balb/c mice were cultured in a horse serum-containing medium on embryonic fibroblast monolayer .
	manualset3
106578	1	402674	5	NULL	NULL	0	NULL	Mast cell degranulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mast cell degranulation ( i.e. the shedding of intact granules ) and vacuolation were examined with the electron microscope .
	manualset3
106579	2	402674	5	NULL	NULL	NULL	NULL	intact granules	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mast cell degranulation ( i.e. the shedding of intact granules ) and vacuolation were examined with the electron microscope .
	manualset3
106580	3	402674	5	NULL	NULL	0	NULL	vacuolation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mast cell degranulation ( i.e. the shedding of intact granules ) and vacuolation were examined with the electron microscope .
	manualset3
106581	4	402674	5	NULL	NULL	0	NULL	electron microscope	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Mast cell degranulation ( i.e. the shedding of intact granules ) and vacuolation were examined with the electron microscope .
	manualset3
106582	1	402675	5	NULL	NULL	0	NULL	Material 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Material contained 40 patients / 28 men and 12 women / mean age 53 + / - 16 years / which died in The Hospital of Lung Diseases in Ld .
	manualset3
106583	2	402675	5	NULL	NULL	0	NULL	40 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Material contained 40 patients / 28 men and 12 women / mean age 53 + / - 16 years / which died in The Hospital of Lung Diseases in Ld .
	manualset3
106584	3	402675	5	NULL	NULL	0	NULL	28 men 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Material contained 40 patients / 28 men and 12 women / mean age 53 + / - 16 years / which died in The Hospital of Lung Diseases in Ld .
	manualset3
106585	4	402675	5	NULL	NULL	0	NULL	12 women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Material contained 40 patients / 28 men and 12 women / mean age 53 + / - 16 years / which died in The Hospital of Lung Diseases in Ld .
	manualset3
106586	5	402675	5	NULL	NULL	0	NULL	mean age 53 + / - 16 years	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Material contained 40 patients / 28 men and 12 women / mean age 53 + / - 16 years / which died in The Hospital of Lung Diseases in Ld .
	manualset3
106587	6	402675	5	NULL	NULL	0	NULL	The Hospital of Lung Diseases	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Material contained 40 patients / 28 men and 12 women / mean age 53 + / - 16 years / which died in The Hospital of Lung Diseases in Ld .
	manualset3
106588	7	402675	5	NULL	NULL	0	NULL	Ld	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Material contained 40 patients / 28 men and 12 women / mean age 53 + / - 16 years / which died in The Hospital of Lung Diseases in Ld .
	manualset3
106589	1	402676	5	NULL	NULL	0	NULL	Materials 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Materials and Methods : Animal experiments were approved by the institutional animal care committee .
	manualset3
106590	2	402676	5	NULL	NULL	0	NULL	Methods 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Materials and Methods : Animal experiments were approved by the institutional animal care committee .
	manualset3
106591	3	402676	5	NULL	NULL	0	NULL	Animal experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Materials and Methods : Animal experiments were approved by the institutional animal care committee .
	manualset3
106592	4	402676	5	NULL	NULL	0	NULL	institutional animal care committee	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Materials and Methods : Animal experiments were approved by the institutional animal care committee .
	manualset3
106593	1	402677	5	NULL	NULL	0	NULL	Maternal concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Maternal concentrations of cotinine and NNAL were measured in urine of the mother and the first urine of her newborn infant by liquid chromatography tandem mass spectrometry ( LC/MS/MS ) .
	manualset3
106594	2	402677	5	NULL	NULL	0	NULL	cotinine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Maternal concentrations of cotinine and NNAL were measured in urine of the mother and the first urine of her newborn infant by liquid chromatography tandem mass spectrometry ( LC/MS/MS ) .
	manualset3
106595	3	402677	5	NULL	NULL	0	NULL	NNAL 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Maternal concentrations of cotinine and NNAL were measured in urine of the mother and the first urine of her newborn infant by liquid chromatography tandem mass spectrometry ( LC/MS/MS ) .
	manualset3
106596	4	402677	5	NULL	NULL	0	NULL	urine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Maternal concentrations of cotinine and NNAL were measured in urine of the mother and the first urine of her newborn infant by liquid chromatography tandem mass spectrometry ( LC/MS/MS ) .
	manualset3
106597	5	402677	5	NULL	NULL	0	NULL	mother 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Maternal concentrations of cotinine and NNAL were measured in urine of the mother and the first urine of her newborn infant by liquid chromatography tandem mass spectrometry ( LC/MS/MS ) .
	manualset3
106598	6	402677	5	NULL	NULL	0	NULL	first urine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Maternal concentrations of cotinine and NNAL were measured in urine of the mother and the first urine of her newborn infant by liquid chromatography tandem mass spectrometry ( LC/MS/MS ) .
	manualset3
106599	7	402677	5	NULL	NULL	0	NULL	newborn infant	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Maternal concentrations of cotinine and NNAL were measured in urine of the mother and the first urine of her newborn infant by liquid chromatography tandem mass spectrometry ( LC/MS/MS ) .
	manualset3
106600	8	402677	5	NULL	NULL	0	NULL	liquid chromatography tandem mass spectrometry ( LC/MS/MS )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Maternal concentrations of cotinine and NNAL were measured in urine of the mother and the first urine of her newborn infant by liquid chromatography tandem mass spectrometry ( LC/MS/MS ) .
	manualset3
106601	1	402678	5	NULL	NULL	0	NULL	Maternal mortality	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Maternal mortality in Australia 1964-72 .
	manualset3
106602	2	402678	5	NULL	NULL	0	NULL	Australia 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Maternal mortality in Australia 1964-72 .
	manualset3
106603	3	402678	5	NULL	NULL	0	NULL	1964-72	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Maternal mortality in Australia 1964-72 .
	manualset3
106604	1	402679	5	NULL	NULL	0	NULL	Mathematical model computations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mathematical model computations predicted hysteresis loops of the instantaneous CO2-HCO ( -3 ) - H + relationship and in vivo blood PCO2-pH relationship due to the finite reaction times for CO2-HCO ( -3 ) - H + reactions .
	manualset3
106605	2	402679	5	NULL	NULL	0	NULL	hysteresis loops	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Mathematical model computations predicted hysteresis loops of the instantaneous CO2-HCO ( -3 ) - H + relationship and in vivo blood PCO2-pH relationship due to the finite reaction times for CO2-HCO ( -3 ) - H + reactions .
	manualset3
106606	3	402679	5	NULL	NULL	0	NULL	CO2-HCO ( -3 ) - H + relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Mathematical model computations predicted hysteresis loops of the instantaneous CO2-HCO ( -3 ) - H + relationship and in vivo blood PCO2-pH relationship due to the finite reaction times for CO2-HCO ( -3 ) - H + reactions .
	manualset3
106607	4	402679	5	NULL	NULL	0	NULL	blood PCO2-pH relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Mathematical model computations predicted hysteresis loops of the instantaneous CO2-HCO ( -3 ) - H + relationship and in vivo blood PCO2-pH relationship due to the finite reaction times for CO2-HCO ( -3 ) - H + reactions .
	manualset3
106608	5	402679	5	NULL	NULL	0	NULL	finite reaction times	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mathematical model computations predicted hysteresis loops of the instantaneous CO2-HCO ( -3 ) - H + relationship and in vivo blood PCO2-pH relationship due to the finite reaction times for CO2-HCO ( -3 ) - H + reactions .
	manualset3
106609	6	402679	5	NULL	NULL	0	NULL	CO2-HCO ( -3 ) - H + reactions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mathematical model computations predicted hysteresis loops of the instantaneous CO2-HCO ( -3 ) - H + relationship and in vivo blood PCO2-pH relationship due to the finite reaction times for CO2-HCO ( -3 ) - H + reactions .
	manualset3
106610	1	402680	5	NULL	NULL	0	NULL	Mathematical modelling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mathematical modelling was used to determine beta-cell glucose sensitivity , rate sensitivity and potentiation .
	manualset3
106611	2	402680	5	NULL	NULL	0	NULL	beta-cell glucose sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mathematical modelling was used to determine beta-cell glucose sensitivity , rate sensitivity and potentiation .
	manualset3
106612	3	402680	5	NULL	NULL	0	NULL	rate sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mathematical modelling was used to determine beta-cell glucose sensitivity , rate sensitivity and potentiation .
	manualset3
106613	4	402680	5	NULL	NULL	0	NULL	potentiation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mathematical modelling was used to determine beta-cell glucose sensitivity , rate sensitivity and potentiation .
	manualset3
106614	1	402681	5	NULL	NULL	0	NULL	Mathematically defined decline curves 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Mathematically defined decline curves were established by determining optimal relationships between methamidophos residues and time , using different models .
	manualset3
106615	2	402681	5	NULL	NULL	0	NULL	optimal relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Mathematically defined decline curves were established by determining optimal relationships between methamidophos residues and time , using different models .
	manualset3
106616	3	402681	5	NULL	NULL	0	NULL	methamidophos residues	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Mathematically defined decline curves were established by determining optimal relationships between methamidophos residues and time , using different models .
	manualset3
106617	4	402681	5	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Mathematically defined decline curves were established by determining optimal relationships between methamidophos residues and time , using different models .
	manualset3
106618	5	402681	5	NULL	NULL	0	NULL	models 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Mathematically defined decline curves were established by determining optimal relationships between methamidophos residues and time , using different models .
	manualset3
106619	1	402682	5	NULL	NULL	0	NULL	Matrix-assisted laser-desorption ionization-time-of-flight MS analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Matrix-assisted laser-desorption ionization-time-of-flight MS analysis and experiments with phosphospecific antibodies revealed that PKC epsilon ( 87 ) is phosphorylated at Thr-566 and Ser-703 , and PKC epsilon ( 95 ) is additionally phosphorylated at Ser-729 .
	manualset3
106620	2	402682	5	NULL	NULL	0	NULL	experiments 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Matrix-assisted laser-desorption ionization-time-of-flight MS analysis and experiments with phosphospecific antibodies revealed that PKC epsilon ( 87 ) is phosphorylated at Thr-566 and Ser-703 , and PKC epsilon ( 95 ) is additionally phosphorylated at Ser-729 .
	manualset3
106621	3	402682	5	NULL	NULL	0	NULL	phosphospecific antibodies	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Matrix-assisted laser-desorption ionization-time-of-flight MS analysis and experiments with phosphospecific antibodies revealed that PKC epsilon ( 87 ) is phosphorylated at Thr-566 and Ser-703 , and PKC epsilon ( 95 ) is additionally phosphorylated at Ser-729 .
	manualset3
106622	4	402682	5	NULL	NULL	NULL	NULL	PKC epsilon ( 87 )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Matrix-assisted laser-desorption ionization-time-of-flight MS analysis and experiments with phosphospecific antibodies revealed that PKC epsilon ( 87 ) is phosphorylated at Thr-566 and Ser-703 , and PKC epsilon ( 95 ) is additionally phosphorylated at Ser-729 .
	manualset3
106623	5	402682	5	NULL	NULL	0	NULL	Thr-566	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Matrix-assisted laser-desorption ionization-time-of-flight MS analysis and experiments with phosphospecific antibodies revealed that PKC epsilon ( 87 ) is phosphorylated at Thr-566 and Ser-703 , and PKC epsilon ( 95 ) is additionally phosphorylated at Ser-729 .
	manualset3
106624	6	402682	5	NULL	NULL	0	NULL	Ser-703	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Matrix-assisted laser-desorption ionization-time-of-flight MS analysis and experiments with phosphospecific antibodies revealed that PKC epsilon ( 87 ) is phosphorylated at Thr-566 and Ser-703 , and PKC epsilon ( 95 ) is additionally phosphorylated at Ser-729 .
	manualset3
106625	7	402682	5	NULL	NULL	0	NULL	PKC epsilon ( 95 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Matrix-assisted laser-desorption ionization-time-of-flight MS analysis and experiments with phosphospecific antibodies revealed that PKC epsilon ( 87 ) is phosphorylated at Thr-566 and Ser-703 , and PKC epsilon ( 95 ) is additionally phosphorylated at Ser-729 .
	manualset3
106626	8	402682	5	NULL	NULL	0	NULL	Ser-729	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Matrix-assisted laser-desorption ionization-time-of-flight MS analysis and experiments with phosphospecific antibodies revealed that PKC epsilon ( 87 ) is phosphorylated at Thr-566 and Ser-703 , and PKC epsilon ( 95 ) is additionally phosphorylated at Ser-729 .
	manualset3
106627	1	402683	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Basic results of the control of the most frequently occurring infections in the Uzbek SSR during the 50 years of Soviet power ) .
	manualset3
106628	2	402683	5	NULL	NULL	0	NULL	frequently occurring infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Basic results of the control of the most frequently occurring infections in the Uzbek SSR during the 50 years of Soviet power ) .
	manualset3
106629	3	402683	5	NULL	NULL	0	NULL	Uzbek SSR	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Basic results of the control of the most frequently occurring infections in the Uzbek SSR during the 50 years of Soviet power ) .
	manualset3
106630	4	402683	5	NULL	NULL	0	NULL	50 years	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	( Basic results of the control of the most frequently occurring infections in the Uzbek SSR during the 50 years of Soviet power ) .
	manualset3
106631	5	402683	5	NULL	NULL	0	NULL	Soviet power 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Basic results of the control of the most frequently occurring infections in the Uzbek SSR during the 50 years of Soviet power ) .
	manualset3
106632	1	402684	5	NULL	NULL	0	NULL	temperature-induced helix-coli transition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A `` normal '' temperature-induced helix-coli transition of poly-gamma-N-carbobenzoxy-L-alpha , gamma-diaminobutyric acid in mixed organic solvents .
	manualset3
106633	2	402684	5	NULL	NULL	0	NULL	poly-gamma-N-carbobenzoxy-L-alpha , gamma-diaminobutyric acid	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A `` normal '' temperature-induced helix-coli transition of poly-gamma-N-carbobenzoxy-L-alpha , gamma-diaminobutyric acid in mixed organic solvents .
	manualset3
106634	3	402684	5	NULL	NULL	0	NULL	mixed organic solvents	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A `` normal '' temperature-induced helix-coli transition of poly-gamma-N-carbobenzoxy-L-alpha , gamma-diaminobutyric acid in mixed organic solvents .
	manualset3
106635	1	402685	5	NULL	NULL	0	NULL	Matrix metalloproteinases ( MMPs )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Matrix metalloproteinases ( MMPs ) have a central role in tumor initiation , invasion and metastasis .
	manualset3
106636	2	402685	5	NULL	NULL	0	NULL	central role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Matrix metalloproteinases ( MMPs ) have a central role in tumor initiation , invasion and metastasis .
	manualset3
106637	3	402685	5	NULL	NULL	0	NULL	tumor initiation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Matrix metalloproteinases ( MMPs ) have a central role in tumor initiation , invasion and metastasis .
	manualset3
106638	4	402685	5	NULL	NULL	0	NULL	tumor invasion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Matrix metalloproteinases ( MMPs ) have a central role in tumor initiation , invasion and metastasis .
	manualset3
106639	5	402685	5	NULL	NULL	0	NULL	metastasis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Matrix metalloproteinases ( MMPs ) have a central role in tumor initiation , invasion and metastasis .
	manualset3
106640	1	402686	5	NULL	NULL	0	NULL	Maturation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Maturation , cytokine production and internalization of B. pseudomallei by BMDC was assessed in response to infection with a highly virulent and a low-virulent clinical isolate .
	manualset3
106641	2	402686	5	NULL	NULL	0	NULL	cytokine production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Maturation , cytokine production and internalization of B. pseudomallei by BMDC was assessed in response to infection with a highly virulent and a low-virulent clinical isolate .
	manualset3
106642	3	402686	5	NULL	NULL	NULL	NULL	internalization 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Maturation , cytokine production and internalization of B. pseudomallei by BMDC was assessed in response to infection with a highly virulent and a low-virulent clinical isolate .
	manualset3
106643	4	402686	5	NULL	NULL	0	NULL	B. pseudomallei 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Maturation , cytokine production and internalization of B. pseudomallei by BMDC was assessed in response to infection with a highly virulent and a low-virulent clinical isolate .
	manualset3
106644	5	402686	5	NULL	NULL	0	NULL	BMDC 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Maturation , cytokine production and internalization of B. pseudomallei by BMDC was assessed in response to infection with a highly virulent and a low-virulent clinical isolate .
	manualset3
106645	6	402686	5	NULL	NULL	0	NULL	response 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Maturation , cytokine production and internalization of B. pseudomallei by BMDC was assessed in response to infection with a highly virulent and a low-virulent clinical isolate .
	manualset3
106646	7	402686	5	NULL	NULL	0	NULL	highly virulent clinical isolate	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Maturation , cytokine production and internalization of B. pseudomallei by BMDC was assessed in response to infection with a highly virulent and a low-virulent clinical isolate .
	manualset3
106647	8	402686	5	NULL	NULL	0	NULL	low-virulent clinical isolate	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Maturation , cytokine production and internalization of B. pseudomallei by BMDC was assessed in response to infection with a highly virulent and a low-virulent clinical isolate .
	manualset3
106649	1	402687	5	NULL	NULL	0	NULL	Maturation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Maturation of bursal stem cells within allogeneic or syngeneic bursal microenvironment : surface determinants and capacity for germinal center formation .
	manualset3
106650	2	402687	5	NULL	NULL	0	NULL	bursal stem cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Maturation of bursal stem cells within allogeneic or syngeneic bursal microenvironment : surface determinants and capacity for germinal center formation .
	manualset3
106651	3	402687	5	NULL	NULL	0	NULL	allogeneic or syngeneic bursal microenvironment	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Maturation of bursal stem cells within allogeneic or syngeneic bursal microenvironment : surface determinants and capacity for germinal center formation .
	manualset3
106652	4	402687	5	NULL	NULL	0	NULL	surface determinants	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Maturation of bursal stem cells within allogeneic or syngeneic bursal microenvironment : surface determinants and capacity for germinal center formation .
	manualset3
106653	5	402687	5	NULL	NULL	0	NULL	capacity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Maturation of bursal stem cells within allogeneic or syngeneic bursal microenvironment : surface determinants and capacity for germinal center formation .
	manualset3
106654	6	402687	5	NULL	NULL	0	NULL	germinal center formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Maturation of bursal stem cells within allogeneic or syngeneic bursal microenvironment : surface determinants and capacity for germinal center formation .
	manualset3
106655	1	402688	5	NULL	NULL	0	NULL	Mature mouse CD4 + T cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mature mouse CD4 + T cells developed in the pig thymus grafts and migrated to the periphery .
	manualset3
106656	2	402688	5	NULL	NULL	0	NULL	pig thymus grafts 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mature mouse CD4 + T cells developed in the pig thymus grafts and migrated to the periphery .
	manualset3
106657	3	402688	5	NULL	NULL	0	NULL	periphery 	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mature mouse CD4 + T cells developed in the pig thymus grafts and migrated to the periphery .
	manualset3
106658	1	402689	5	NULL	NULL	0	NULL	Mature milk	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Mature milk contained more lipids and less protein , whereas the increase of parity number was associated with an increase in lipid concentration .
	manualset3
106659	2	402689	5	NULL	NULL	0	NULL	lipids 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mature milk contained more lipids and less protein , whereas the increase of parity number was associated with an increase in lipid concentration .
	manualset3
106660	3	402689	5	NULL	NULL	0	NULL	protein 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mature milk contained more lipids and less protein , whereas the increase of parity number was associated with an increase in lipid concentration .
	manualset3
106661	4	402689	5	NULL	NULL	0	NULL	parity number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mature milk contained more lipids and less protein , whereas the increase of parity number was associated with an increase in lipid concentration .
	manualset3
106662	5	402689	5	NULL	NULL	0	NULL	lipid concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mature milk contained more lipids and less protein , whereas the increase of parity number was associated with an increase in lipid concentration .
	manualset3
106663	1	402690	5	NULL	NULL	0	NULL	Mature , male chickens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mature , male chickens , Bobwhite quail , and rats differed with respect to glutathione S-transferase ( GST ) activity in the kidney , duodenum and testis , but species differences were not observed in the liver .
	manualset3
106664	2	402690	5	NULL	NULL	0	NULL	Bobwhite quail	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mature , male chickens , Bobwhite quail , and rats differed with respect to glutathione S-transferase ( GST ) activity in the kidney , duodenum and testis , but species differences were not observed in the liver .
	manualset3
106665	3	402690	5	NULL	NULL	0	NULL	rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mature , male chickens , Bobwhite quail , and rats differed with respect to glutathione S-transferase ( GST ) activity in the kidney , duodenum and testis , but species differences were not observed in the liver .
	manualset3
106666	4	402690	5	NULL	NULL	0	NULL	glutathione S-transferase ( GST ) activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mature , male chickens , Bobwhite quail , and rats differed with respect to glutathione S-transferase ( GST ) activity in the kidney , duodenum and testis , but species differences were not observed in the liver .
	manualset3
106667	5	402690	5	NULL	NULL	0	NULL	kidney 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mature , male chickens , Bobwhite quail , and rats differed with respect to glutathione S-transferase ( GST ) activity in the kidney , duodenum and testis , but species differences were not observed in the liver .
	manualset3
106668	6	402690	5	NULL	NULL	0	NULL	duodenum 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mature , male chickens , Bobwhite quail , and rats differed with respect to glutathione S-transferase ( GST ) activity in the kidney , duodenum and testis , but species differences were not observed in the liver .
	manualset3
106669	7	402690	5	NULL	NULL	0	NULL	testis 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mature , male chickens , Bobwhite quail , and rats differed with respect to glutathione S-transferase ( GST ) activity in the kidney , duodenum and testis , but species differences were not observed in the liver .
	manualset3
106670	8	402690	5	NULL	NULL	0	NULL	species differences	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mature , male chickens , Bobwhite quail , and rats differed with respect to glutathione S-transferase ( GST ) activity in the kidney , duodenum and testis , but species differences were not observed in the liver .
	manualset3
106671	9	402690	5	NULL	NULL	0	NULL	liver 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mature , male chickens , Bobwhite quail , and rats differed with respect to glutathione S-transferase ( GST ) activity in the kidney , duodenum and testis , but species differences were not observed in the liver .
	manualset3
106672	1	402691	5	NULL	NULL	0	NULL	Maturity - and sex-related changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Maturity - and sex-related changes in tibial bone geometry , strength and bone-muscle strength indices during growth : a 20-month pQCT study .
	manualset3
106673	2	402691	5	NULL	NULL	NULL	NULL	tibial bone geometry indices 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Maturity - and sex-related changes in tibial bone geometry , strength and bone-muscle strength indices during growth : a 20-month pQCT study .
	manualset3
106674	3	402691	5	NULL	NULL	NULL	NULL	strength indices 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Maturity - and sex-related changes in tibial bone geometry , strength and bone-muscle strength indices during growth : a 20-month pQCT study .
	manualset3
106675	4	402691	5	NULL	NULL	NULL	NULL	bone-muscle strength indices 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Maturity - and sex-related changes in tibial bone geometry , strength and bone-muscle strength indices during growth : a 20-month pQCT study .
	manualset3
106676	5	402691	5	NULL	NULL	0	NULL	20-month	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Maturity - and sex-related changes in tibial bone geometry , strength and bone-muscle strength indices during growth : a 20-month pQCT study .
	manualset3
106677	6	402691	5	NULL	NULL	0	NULL	pQCT study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Maturity - and sex-related changes in tibial bone geometry , strength and bone-muscle strength indices during growth : a 20-month pQCT study .
	manualset3
106678	1	402692	5	NULL	NULL	0	NULL	Maximal MVD	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal MVD proved to be an independent prognostic parameter useful in conjunction with other known prognostic markers in human prostate cancer .
	manualset3
106679	2	402692	5	NULL	NULL	0	NULL	independent prognostic parameter	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal MVD proved to be an independent prognostic parameter useful in conjunction with other known prognostic markers in human prostate cancer .
	manualset3
106680	3	402692	5	NULL	NULL	0	NULL	conjunction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal MVD proved to be an independent prognostic parameter useful in conjunction with other known prognostic markers in human prostate cancer .
	manualset3
106681	4	402692	5	NULL	NULL	0	NULL	prognostic markers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal MVD proved to be an independent prognostic parameter useful in conjunction with other known prognostic markers in human prostate cancer .
	manualset3
106682	5	402692	5	NULL	NULL	0	NULL	human prostate cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal MVD proved to be an independent prognostic parameter useful in conjunction with other known prognostic markers in human prostate cancer .
	manualset3
106683	1	402693	5	NULL	NULL	0	NULL	barium enema	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A barium enema showing a relatively radiolucent mass , caused by the radiolucency of fat , is suggestive of a lipoma .
	manualset3
106684	2	402693	5	NULL	NULL	0	NULL	radiolucent mass	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A barium enema showing a relatively radiolucent mass , caused by the radiolucency of fat , is suggestive of a lipoma .
	manualset3
106685	3	402693	5	NULL	NULL	0	NULL	radiolucency 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A barium enema showing a relatively radiolucent mass , caused by the radiolucency of fat , is suggestive of a lipoma .
	manualset3
106686	4	402693	5	NULL	NULL	0	NULL	fat 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A barium enema showing a relatively radiolucent mass , caused by the radiolucency of fat , is suggestive of a lipoma .
	manualset3
106687	5	402693	5	NULL	NULL	0	NULL	lipoma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A barium enema showing a relatively radiolucent mass , caused by the radiolucency of fat , is suggestive of a lipoma .
	manualset3
106688	1	402694	5	NULL	NULL	NULL	NULL	Maximal force	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Maximal force , endurance , and recovery times of the tongue , electromyogram ( EMG ) absolute value , and EMG spectral analysis of the GGm obtained during submaximal contractions were compared in eight individuals without chronic snoring and eight OSAS patients .
	manualset3
106691	2	402694	5	NULL	NULL	0	NULL	endurance 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal force , endurance , and recovery times of the tongue , electromyogram ( EMG ) absolute value , and EMG spectral analysis of the GGm obtained during submaximal contractions were compared in eight individuals without chronic snoring and eight OSAS patients .
	manualset3
106694	3	402694	5	NULL	NULL	0	NULL	recovery times	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal force , endurance , and recovery times of the tongue , electromyogram ( EMG ) absolute value , and EMG spectral analysis of the GGm obtained during submaximal contractions were compared in eight individuals without chronic snoring and eight OSAS patients .
	manualset3
106695	4	402694	5	NULL	NULL	0	NULL	tongue 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal force , endurance , and recovery times of the tongue , electromyogram ( EMG ) absolute value , and EMG spectral analysis of the GGm obtained during submaximal contractions were compared in eight individuals without chronic snoring and eight OSAS patients .
	manualset3
106696	5	402694	5	NULL	NULL	0	NULL	electromyogram ( EMG ) absolute value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal force , endurance , and recovery times of the tongue , electromyogram ( EMG ) absolute value , and EMG spectral analysis of the GGm obtained during submaximal contractions were compared in eight individuals without chronic snoring and eight OSAS patients .
	manualset3
106698	6	402694	5	NULL	NULL	0	NULL	EMG spectral analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal force , endurance , and recovery times of the tongue , electromyogram ( EMG ) absolute value , and EMG spectral analysis of the GGm obtained during submaximal contractions were compared in eight individuals without chronic snoring and eight OSAS patients .
	manualset3
106700	7	402694	5	NULL	NULL	0	NULL	GGm	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal force , endurance , and recovery times of the tongue , electromyogram ( EMG ) absolute value , and EMG spectral analysis of the GGm obtained during submaximal contractions were compared in eight individuals without chronic snoring and eight OSAS patients .
	manualset3
106702	8	402694	5	NULL	NULL	0	NULL	submaximal contractions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal force , endurance , and recovery times of the tongue , electromyogram ( EMG ) absolute value , and EMG spectral analysis of the GGm obtained during submaximal contractions were compared in eight individuals without chronic snoring and eight OSAS patients .
	manualset3
106704	9	402694	5	NULL	NULL	0	NULL	eight individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal force , endurance , and recovery times of the tongue , electromyogram ( EMG ) absolute value , and EMG spectral analysis of the GGm obtained during submaximal contractions were compared in eight individuals without chronic snoring and eight OSAS patients .
	manualset3
106705	10	402694	5	NULL	NULL	0	NULL	chronic snoring	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal force , endurance , and recovery times of the tongue , electromyogram ( EMG ) absolute value , and EMG spectral analysis of the GGm obtained during submaximal contractions were compared in eight individuals without chronic snoring and eight OSAS patients .
	manualset3
106707	11	402694	5	NULL	NULL	0	NULL	eight OSAS patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal force , endurance , and recovery times of the tongue , electromyogram ( EMG ) absolute value , and EMG spectral analysis of the GGm obtained during submaximal contractions were compared in eight individuals without chronic snoring and eight OSAS patients .
	manualset3
106719	1	402695	5	NULL	NULL	0	NULL	Maximal molar bite force	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal molar bite force , which increased pre-treatment ( T0-T1 ) , decreased during functional appliance treatment ( T1-T2 ) .
	manualset3
106721	2	402695	5	NULL	NULL	0	NULL	pre-treatment ( T0-T1 )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal molar bite force , which increased pre-treatment ( T0-T1 ) , decreased during functional appliance treatment ( T1-T2 ) .
	manualset3
106722	3	402695	5	NULL	NULL	0	NULL	functional appliance treatment ( T1-T2 )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal molar bite force , which increased pre-treatment ( T0-T1 ) , decreased during functional appliance treatment ( T1-T2 ) .
	manualset3
106734	1	402696	5	NULL	NULL	0	NULL	Maximal pacing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal pacing at 275 bpm caused only a moderate flow elevation in control ( 20 + / - 6.8 % ) and CO2 conditions ( 20.3 + / - 4.03 % ) , but marked vasodilation during nitroglycerin infusion ( 85.2 + / - 14.6 % ) .
	manualset3
106735	2	402696	5	NULL	NULL	0	NULL	275 bpm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal pacing at 275 bpm caused only a moderate flow elevation in control ( 20 + / - 6.8 % ) and CO2 conditions ( 20.3 + / - 4.03 % ) , but marked vasodilation during nitroglycerin infusion ( 85.2 + / - 14.6 % ) .
	manualset3
106736	3	402696	5	NULL	NULL	0	NULL	moderate flow elevation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal pacing at 275 bpm caused only a moderate flow elevation in control ( 20 + / - 6.8 % ) and CO2 conditions ( 20.3 + / - 4.03 % ) , but marked vasodilation during nitroglycerin infusion ( 85.2 + / - 14.6 % ) .
	manualset3
106737	4	402696	5	NULL	NULL	0	NULL	 20 + / - 6.8 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal pacing at 275 bpm caused only a moderate flow elevation in control ( 20 + / - 6.8 % ) and CO2 conditions ( 20.3 + / - 4.03 % ) , but marked vasodilation during nitroglycerin infusion ( 85.2 + / - 14.6 % ) .
	manualset3
106738	5	402696	5	NULL	NULL	0	NULL	CO2 conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal pacing at 275 bpm caused only a moderate flow elevation in control ( 20 + / - 6.8 % ) and CO2 conditions ( 20.3 + / - 4.03 % ) , but marked vasodilation during nitroglycerin infusion ( 85.2 + / - 14.6 % ) .
	manualset3
106739	6	402696	5	NULL	NULL	0	NULL	20.3 + / - 4.03 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal pacing at 275 bpm caused only a moderate flow elevation in control ( 20 + / - 6.8 % ) and CO2 conditions ( 20.3 + / - 4.03 % ) , but marked vasodilation during nitroglycerin infusion ( 85.2 + / - 14.6 % ) .
	manualset3
106740	7	402696	5	NULL	NULL	0	NULL	marked vasodilation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal pacing at 275 bpm caused only a moderate flow elevation in control ( 20 + / - 6.8 % ) and CO2 conditions ( 20.3 + / - 4.03 % ) , but marked vasodilation during nitroglycerin infusion ( 85.2 + / - 14.6 % ) .
	manualset3
106741	8	402696	5	NULL	NULL	0	NULL	nitroglycerin infusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal pacing at 275 bpm caused only a moderate flow elevation in control ( 20 + / - 6.8 % ) and CO2 conditions ( 20.3 + / - 4.03 % ) , but marked vasodilation during nitroglycerin infusion ( 85.2 + / - 14.6 % ) .
	manualset3
106742	9	402696	5	NULL	NULL	0	NULL	85.2 + / - 14.6 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal pacing at 275 bpm caused only a moderate flow elevation in control ( 20 + / - 6.8 % ) and CO2 conditions ( 20.3 + / - 4.03 % ) , but marked vasodilation during nitroglycerin infusion ( 85.2 + / - 14.6 % ) .
	manualset3
106743	1	402697	5	NULL	NULL	0	NULL	Maximum contact pressure	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximum contact pressure on the metal-bone interface similarly changed and shifted from the lateral edge to the medial edge of the implant as the inclination changed to varus .
	manualset3
106744	2	402697	5	NULL	NULL	0	NULL	metal-bone interface	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximum contact pressure on the metal-bone interface similarly changed and shifted from the lateral edge to the medial edge of the implant as the inclination changed to varus .
	manualset3
106745	3	402697	5	NULL	NULL	NULL	NULL	lateral edge	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Maximum contact pressure on the metal-bone interface similarly changed and shifted from the lateral edge to the medial edge of the implant as the inclination changed to varus .
	manualset3
106746	4	402697	5	NULL	NULL	0	NULL	medial edge 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximum contact pressure on the metal-bone interface similarly changed and shifted from the lateral edge to the medial edge of the implant as the inclination changed to varus .
	manualset3
106747	5	402697	5	NULL	NULL	0	NULL	implant 	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximum contact pressure on the metal-bone interface similarly changed and shifted from the lateral edge to the medial edge of the implant as the inclination changed to varus .
	manualset3
106748	6	402697	5	NULL	NULL	0	NULL	inclination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximum contact pressure on the metal-bone interface similarly changed and shifted from the lateral edge to the medial edge of the implant as the inclination changed to varus .
	manualset3
106749	7	402697	5	NULL	NULL	0	NULL	varus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximum contact pressure on the metal-bone interface similarly changed and shifted from the lateral edge to the medial edge of the implant as the inclination changed to varus .
	manualset3
106750	1	402698	5	NULL	NULL	0	NULL	Mb oxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mb oxidation can proceed rapidly ( within 15 min ) in the presence of iron and the absence of lipid , especially if reducing compounds such as rosmarinic acid or eugenol are also present to maintain iron in an active ferrous form .
	manualset3
106751	2	402698	5	NULL	NULL	0	NULL	15 min	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Mb oxidation can proceed rapidly ( within 15 min ) in the presence of iron and the absence of lipid , especially if reducing compounds such as rosmarinic acid or eugenol are also present to maintain iron in an active ferrous form .
	manualset3
106752	3	402698	5	NULL	NULL	0	NULL	iron 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Mb oxidation can proceed rapidly ( within 15 min ) in the presence of iron and the absence of lipid , especially if reducing compounds such as rosmarinic acid or eugenol are also present to maintain iron in an active ferrous form .
	manualset3
106753	4	402698	5	NULL	NULL	0	NULL	lipid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mb oxidation can proceed rapidly ( within 15 min ) in the presence of iron and the absence of lipid , especially if reducing compounds such as rosmarinic acid or eugenol are also present to maintain iron in an active ferrous form .
	manualset3
106754	5	402698	5	NULL	NULL	0	NULL	reducing compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mb oxidation can proceed rapidly ( within 15 min ) in the presence of iron and the absence of lipid , especially if reducing compounds such as rosmarinic acid or eugenol are also present to maintain iron in an active ferrous form .
	manualset3
106755	6	402698	5	NULL	NULL	0	NULL	rosmarinic acid	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Mb oxidation can proceed rapidly ( within 15 min ) in the presence of iron and the absence of lipid , especially if reducing compounds such as rosmarinic acid or eugenol are also present to maintain iron in an active ferrous form .
	manualset3
106756	7	402698	5	NULL	NULL	0	NULL	eugenol 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Mb oxidation can proceed rapidly ( within 15 min ) in the presence of iron and the absence of lipid , especially if reducing compounds such as rosmarinic acid or eugenol are also present to maintain iron in an active ferrous form .
	manualset3
106757	8	402698	5	NULL	NULL	0	NULL	iron 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Mb oxidation can proceed rapidly ( within 15 min ) in the presence of iron and the absence of lipid , especially if reducing compounds such as rosmarinic acid or eugenol are also present to maintain iron in an active ferrous form .
	manualset3
106758	9	402698	5	NULL	NULL	0	NULL	active ferrous form	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Mb oxidation can proceed rapidly ( within 15 min ) in the presence of iron and the absence of lipid , especially if reducing compounds such as rosmarinic acid or eugenol are also present to maintain iron in an active ferrous form .
	manualset3
106759	1	402699	5	NULL	NULL	0	NULL	Mc-ab 1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mc-ab 1 , which was raised against growth hormone but cross-reacted with human placental lactogen yielded higher GH immunoreactivity levels in serum than one based on a polyclonal antiserum .
	manualset3
106760	2	402699	5	NULL	NULL	0	NULL	growth hormone	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mc-ab 1 , which was raised against growth hormone but cross-reacted with human placental lactogen yielded higher GH immunoreactivity levels in serum than one based on a polyclonal antiserum .
	manualset3
106761	3	402699	5	NULL	NULL	0	NULL	human placental lactogen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mc-ab 1 , which was raised against growth hormone but cross-reacted with human placental lactogen yielded higher GH immunoreactivity levels in serum than one based on a polyclonal antiserum .
	manualset3
106762	4	402699	5	NULL	NULL	0	NULL	higher GH immunoreactivity levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mc-ab 1 , which was raised against growth hormone but cross-reacted with human placental lactogen yielded higher GH immunoreactivity levels in serum than one based on a polyclonal antiserum .
	manualset3
106763	5	402699	5	NULL	NULL	0	NULL	serum 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Mc-ab 1 , which was raised against growth hormone but cross-reacted with human placental lactogen yielded higher GH immunoreactivity levels in serum than one based on a polyclonal antiserum .
	manualset3
106764	6	402699	5	NULL	NULL	0	NULL	polyclonal antiserum	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Mc-ab 1 , which was raised against growth hormone but cross-reacted with human placental lactogen yielded higher GH immunoreactivity levels in serum than one based on a polyclonal antiserum .
	manualset3
106765	1	402700	5	NULL	NULL	0	NULL	change 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Me ) tended to be more reproducible and more sensitive to change ( SRM up to -0.62 ) than cartilage volume ( SRM up to -0.44 ) , cartilage thickness over the cartilaginous area ( ThCcAB ; SRM up to -0.48 ) or maximum cartilage thickness ( ThCtAB ; SRM up to -0.35 ) .
	manualset3
106766	2	402700	5	NULL	NULL	0	NULL	SRM up to -0.62	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Me ) tended to be more reproducible and more sensitive to change ( SRM up to -0.62 ) than cartilage volume ( SRM up to -0.44 ) , cartilage thickness over the cartilaginous area ( ThCcAB ; SRM up to -0.48 ) or maximum cartilage thickness ( ThCtAB ; SRM up to -0.35 ) .
	manualset3
106767	3	402700	5	NULL	NULL	0	NULL	cartilage volume	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Me ) tended to be more reproducible and more sensitive to change ( SRM up to -0.62 ) than cartilage volume ( SRM up to -0.44 ) , cartilage thickness over the cartilaginous area ( ThCcAB ; SRM up to -0.48 ) or maximum cartilage thickness ( ThCtAB ; SRM up to -0.35 ) .
	manualset3
106768	4	402700	5	NULL	NULL	0	NULL	SRM up to -0.44	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Me ) tended to be more reproducible and more sensitive to change ( SRM up to -0.62 ) than cartilage volume ( SRM up to -0.44 ) , cartilage thickness over the cartilaginous area ( ThCcAB ; SRM up to -0.48 ) or maximum cartilage thickness ( ThCtAB ; SRM up to -0.35 ) .
	manualset3
106769	5	402700	5	NULL	NULL	0	NULL	cartilage thickness	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Me ) tended to be more reproducible and more sensitive to change ( SRM up to -0.62 ) than cartilage volume ( SRM up to -0.44 ) , cartilage thickness over the cartilaginous area ( ThCcAB ; SRM up to -0.48 ) or maximum cartilage thickness ( ThCtAB ; SRM up to -0.35 ) .
	manualset3
106770	6	402700	5	NULL	NULL	0	NULL	cartilaginous area	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Me ) tended to be more reproducible and more sensitive to change ( SRM up to -0.62 ) than cartilage volume ( SRM up to -0.44 ) , cartilage thickness over the cartilaginous area ( ThCcAB ; SRM up to -0.48 ) or maximum cartilage thickness ( ThCtAB ; SRM up to -0.35 ) .
	manualset3
106771	7	402700	5	NULL	NULL	0	NULL	ThCcAB 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Me ) tended to be more reproducible and more sensitive to change ( SRM up to -0.62 ) than cartilage volume ( SRM up to -0.44 ) , cartilage thickness over the cartilaginous area ( ThCcAB ; SRM up to -0.48 ) or maximum cartilage thickness ( ThCtAB ; SRM up to -0.35 ) .
	manualset3
106772	8	402700	5	NULL	NULL	0	NULL	SRM up to -0.48	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Me ) tended to be more reproducible and more sensitive to change ( SRM up to -0.62 ) than cartilage volume ( SRM up to -0.44 ) , cartilage thickness over the cartilaginous area ( ThCcAB ; SRM up to -0.48 ) or maximum cartilage thickness ( ThCtAB ; SRM up to -0.35 ) .
	manualset3
106773	9	402700	5	NULL	NULL	0	NULL	maximum cartilage thickness	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Me ) tended to be more reproducible and more sensitive to change ( SRM up to -0.62 ) than cartilage volume ( SRM up to -0.44 ) , cartilage thickness over the cartilaginous area ( ThCcAB ; SRM up to -0.48 ) or maximum cartilage thickness ( ThCtAB ; SRM up to -0.35 ) .
	manualset3
106774	10	402700	5	NULL	NULL	0	NULL	ThCtAB 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Me ) tended to be more reproducible and more sensitive to change ( SRM up to -0.62 ) than cartilage volume ( SRM up to -0.44 ) , cartilage thickness over the cartilaginous area ( ThCcAB ; SRM up to -0.48 ) or maximum cartilage thickness ( ThCtAB ; SRM up to -0.35 ) .
	manualset3
106775	11	402700	5	NULL	NULL	0	NULL	SRM up to -0.35	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Me ) tended to be more reproducible and more sensitive to change ( SRM up to -0.62 ) than cartilage volume ( SRM up to -0.44 ) , cartilage thickness over the cartilaginous area ( ThCcAB ; SRM up to -0.48 ) or maximum cartilage thickness ( ThCtAB ; SRM up to -0.35 ) .
	manualset3
106776	1	402701	5	NULL	NULL	0	NULL	Mean CSF AChE activity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean CSF AChE activity in PSP subjects was significantly reduced by 31 % relative to control subjects ( p less than 0.002 ) .
	manualset3
106777	2	402701	5	NULL	NULL	0	NULL	PSP subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean CSF AChE activity in PSP subjects was significantly reduced by 31 % relative to control subjects ( p less than 0.002 ) .
	manualset3
106778	3	402701	5	NULL	NULL	0	NULL	31 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean CSF AChE activity in PSP subjects was significantly reduced by 31 % relative to control subjects ( p less than 0.002 ) .
	manualset3
106779	4	402701	5	NULL	NULL	0	NULL	control subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean CSF AChE activity in PSP subjects was significantly reduced by 31 % relative to control subjects ( p less than 0.002 ) .
	manualset3
106780	5	402701	5	NULL	NULL	0	NULL	p less than 0.002	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean CSF AChE activity in PSP subjects was significantly reduced by 31 % relative to control subjects ( p less than 0.002 ) .
	manualset3
106781	1	402702	5	NULL	NULL	0	NULL	bench scale study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A bench scale study was carried out in order to evaluate the applicability of dissolved air flotation ( DAF ) as an advanced treatment for effluents from three different domestic wastewater treatment processes , namely : ( i ) a tertiary activated sludge plant ; ( ii ) an upflow sludge blanket anaerobic reactor ( UASB ) ; and ( iii ) a high-rate stabilization pond .
	manualset3
106782	2	402702	5	NULL	NULL	0	NULL	evaluate 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A bench scale study was carried out in order to evaluate the applicability of dissolved air flotation ( DAF ) as an advanced treatment for effluents from three different domestic wastewater treatment processes , namely : ( i ) a tertiary activated sludge plant ; ( ii ) an upflow sludge blanket anaerobic reactor ( UASB ) ; and ( iii ) a high-rate stabilization pond .
	manualset3
106783	3	402702	5	NULL	NULL	0	NULL	applicability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A bench scale study was carried out in order to evaluate the applicability of dissolved air flotation ( DAF ) as an advanced treatment for effluents from three different domestic wastewater treatment processes , namely : ( i ) a tertiary activated sludge plant ; ( ii ) an upflow sludge blanket anaerobic reactor ( UASB ) ; and ( iii ) a high-rate stabilization pond .
	manualset3
106784	4	402702	5	NULL	NULL	0	NULL	dissolved air flotation ( DAF )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A bench scale study was carried out in order to evaluate the applicability of dissolved air flotation ( DAF ) as an advanced treatment for effluents from three different domestic wastewater treatment processes , namely : ( i ) a tertiary activated sludge plant ; ( ii ) an upflow sludge blanket anaerobic reactor ( UASB ) ; and ( iii ) a high-rate stabilization pond .
	manualset3
106785	5	402702	5	NULL	NULL	NULL	NULL	advanced treatment	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A bench scale study was carried out in order to evaluate the applicability of dissolved air flotation ( DAF ) as an advanced treatment for effluents from three different domestic wastewater treatment processes , namely : ( i ) a tertiary activated sludge plant ; ( ii ) an upflow sludge blanket anaerobic reactor ( UASB ) ; and ( iii ) a high-rate stabilization pond .
	manualset3
106786	6	402702	5	NULL	NULL	0	NULL	effluents 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A bench scale study was carried out in order to evaluate the applicability of dissolved air flotation ( DAF ) as an advanced treatment for effluents from three different domestic wastewater treatment processes , namely : ( i ) a tertiary activated sludge plant ; ( ii ) an upflow sludge blanket anaerobic reactor ( UASB ) ; and ( iii ) a high-rate stabilization pond .
	manualset3
106787	7	402702	5	NULL	NULL	0	NULL	domestic wastewater treatment processes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A bench scale study was carried out in order to evaluate the applicability of dissolved air flotation ( DAF ) as an advanced treatment for effluents from three different domestic wastewater treatment processes , namely : ( i ) a tertiary activated sludge plant ; ( ii ) an upflow sludge blanket anaerobic reactor ( UASB ) ; and ( iii ) a high-rate stabilization pond .
	manualset3
106788	8	402702	5	NULL	NULL	0	NULL	tertiary activated sludge plant	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A bench scale study was carried out in order to evaluate the applicability of dissolved air flotation ( DAF ) as an advanced treatment for effluents from three different domestic wastewater treatment processes , namely : ( i ) a tertiary activated sludge plant ; ( ii ) an upflow sludge blanket anaerobic reactor ( UASB ) ; and ( iii ) a high-rate stabilization pond .
	manualset3
106789	9	402702	5	NULL	NULL	0	NULL	upflow sludge blanket anaerobic reactor ( UASB )	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A bench scale study was carried out in order to evaluate the applicability of dissolved air flotation ( DAF ) as an advanced treatment for effluents from three different domestic wastewater treatment processes , namely : ( i ) a tertiary activated sludge plant ; ( ii ) an upflow sludge blanket anaerobic reactor ( UASB ) ; and ( iii ) a high-rate stabilization pond .
	manualset3
106790	10	402702	5	NULL	NULL	0	NULL	high-rate stabilization pond	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A bench scale study was carried out in order to evaluate the applicability of dissolved air flotation ( DAF ) as an advanced treatment for effluents from three different domestic wastewater treatment processes , namely : ( i ) a tertiary activated sludge plant ; ( ii ) an upflow sludge blanket anaerobic reactor ( UASB ) ; and ( iii ) a high-rate stabilization pond .
	manualset3
106791	1	402703	5	NULL	NULL	0	NULL	Mean attenuation	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean attenuation for the three protocols was measured in the superior vena cava , pulmonary trunk , ascending aorta , and descending aorta .
	manualset3
106792	2	402703	5	NULL	NULL	0	NULL	protocols 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean attenuation for the three protocols was measured in the superior vena cava , pulmonary trunk , ascending aorta , and descending aorta .
	manualset3
106793	3	402703	5	NULL	NULL	0	NULL	superior vena cava	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean attenuation for the three protocols was measured in the superior vena cava , pulmonary trunk , ascending aorta , and descending aorta .
	manualset3
106794	4	402703	5	NULL	NULL	0	NULL	pulmonary trunk	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean attenuation for the three protocols was measured in the superior vena cava , pulmonary trunk , ascending aorta , and descending aorta .
	manualset3
106795	5	402703	5	NULL	NULL	0	NULL	ascending aorta	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean attenuation for the three protocols was measured in the superior vena cava , pulmonary trunk , ascending aorta , and descending aorta .
	manualset3
106796	6	402703	5	NULL	NULL	0	NULL	descending aorta	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean attenuation for the three protocols was measured in the superior vena cava , pulmonary trunk , ascending aorta , and descending aorta .
	manualset3
106797	1	402704	5	NULL	NULL	0	NULL	Mean daily dose 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean daily dose ( 19.4 + / -11.4 , 16.3 + / -12.1 , and 11.3 + / -7.6 mg/kg/day ; p = 0.003 ) and total VPA concentration ( 56.4 + / -25.8 , 47.7 + / -22.6 , and 38.7 + / -23.1 mg/kg/day ; p = 0.003 ) decreased by age groups ( 65-74 , 75-84 , and ) or = 85 years ) .
	manualset3
106798	2	402704	5	NULL	NULL	0	NULL	19.4 + / -11.4 , 16.3 + / -12.1 , and 11.3 + / -7.6 mg/kg/day 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean daily dose ( 19.4 + / -11.4 , 16.3 + / -12.1 , and 11.3 + / -7.6 mg/kg/day ; p = 0.003 ) and total VPA concentration ( 56.4 + / -25.8 , 47.7 + / -22.6 , and 38.7 + / -23.1 mg/kg/day ; p = 0.003 ) decreased by age groups ( 65-74 , 75-84 , and ) or = 85 years ) .
	manualset3
106799	3	402704	5	NULL	NULL	0	NULL	p = 0.003	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean daily dose ( 19.4 + / -11.4 , 16.3 + / -12.1 , and 11.3 + / -7.6 mg/kg/day ; p = 0.003 ) and total VPA concentration ( 56.4 + / -25.8 , 47.7 + / -22.6 , and 38.7 + / -23.1 mg/kg/day ; p = 0.003 ) decreased by age groups ( 65-74 , 75-84 , and ) or = 85 years ) .
	manualset3
106800	4	402704	5	NULL	NULL	0	NULL	total VPA concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean daily dose ( 19.4 + / -11.4 , 16.3 + / -12.1 , and 11.3 + / -7.6 mg/kg/day ; p = 0.003 ) and total VPA concentration ( 56.4 + / -25.8 , 47.7 + / -22.6 , and 38.7 + / -23.1 mg/kg/day ; p = 0.003 ) decreased by age groups ( 65-74 , 75-84 , and ) or = 85 years ) .
	manualset3
106801	5	402704	5	NULL	NULL	0	NULL	56.4 + / -25.8 , 47.7 + / -22.6 , and 38.7 + / -23.1 mg/kg/day	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean daily dose ( 19.4 + / -11.4 , 16.3 + / -12.1 , and 11.3 + / -7.6 mg/kg/day ; p = 0.003 ) and total VPA concentration ( 56.4 + / -25.8 , 47.7 + / -22.6 , and 38.7 + / -23.1 mg/kg/day ; p = 0.003 ) decreased by age groups ( 65-74 , 75-84 , and ) or = 85 years ) .
	manualset3
106802	6	402704	5	NULL	NULL	0	NULL	p = 0.003	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean daily dose ( 19.4 + / -11.4 , 16.3 + / -12.1 , and 11.3 + / -7.6 mg/kg/day ; p = 0.003 ) and total VPA concentration ( 56.4 + / -25.8 , 47.7 + / -22.6 , and 38.7 + / -23.1 mg/kg/day ; p = 0.003 ) decreased by age groups ( 65-74 , 75-84 , and ) or = 85 years ) .
	manualset3
106803	7	402704	5	NULL	NULL	0	NULL	age groups 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean daily dose ( 19.4 + / -11.4 , 16.3 + / -12.1 , and 11.3 + / -7.6 mg/kg/day ; p = 0.003 ) and total VPA concentration ( 56.4 + / -25.8 , 47.7 + / -22.6 , and 38.7 + / -23.1 mg/kg/day ; p = 0.003 ) decreased by age groups ( 65-74 , 75-84 , and ) or = 85 years ) .
	manualset3
106804	8	402704	5	NULL	NULL	0	NULL	65-74 , 75-84 , and ) or = 85 years	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean daily dose ( 19.4 + / -11.4 , 16.3 + / -12.1 , and 11.3 + / -7.6 mg/kg/day ; p = 0.003 ) and total VPA concentration ( 56.4 + / -25.8 , 47.7 + / -22.6 , and 38.7 + / -23.1 mg/kg/day ; p = 0.003 ) decreased by age groups ( 65-74 , 75-84 , and ) or = 85 years ) .
	manualset3
106805	1	402705	5	NULL	NULL	0	NULL	mitral poppet diameter 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean decrease in mitral poppet diameter was 0.4 % ( range 0 % to 1.5 % ) , in contrast to a mean of 5.8 % for aortic poppets .
	manualset3
106806	2	402705	5	NULL	NULL	0	NULL	0.4 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean decrease in mitral poppet diameter was 0.4 % ( range 0 % to 1.5 % ) , in contrast to a mean of 5.8 % for aortic poppets .
	manualset3
106807	3	402705	5	NULL	NULL	0	NULL	range 0 % to 1.5 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean decrease in mitral poppet diameter was 0.4 % ( range 0 % to 1.5 % ) , in contrast to a mean of 5.8 % for aortic poppets .
	manualset3
106808	4	402705	5	NULL	NULL	0	NULL	mean 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean decrease in mitral poppet diameter was 0.4 % ( range 0 % to 1.5 % ) , in contrast to a mean of 5.8 % for aortic poppets .
	manualset3
106809	5	402705	5	NULL	NULL	0	NULL	5.8 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean decrease in mitral poppet diameter was 0.4 % ( range 0 % to 1.5 % ) , in contrast to a mean of 5.8 % for aortic poppets .
	manualset3
106810	6	402705	5	NULL	NULL	0	NULL	aortic poppets	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean decrease in mitral poppet diameter was 0.4 % ( range 0 % to 1.5 % ) , in contrast to a mean of 5.8 % for aortic poppets .
	manualset3
106811	1	402706	5	NULL	NULL	0	NULL	24.4 months	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean follow-up was 24.4 months ( range : 6-49 months ) ; 10 patients were lost to follow-up .
	manualset3
106812	2	402706	5	NULL	NULL	0	NULL	 range : 6-49 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean follow-up was 24.4 months ( range : 6-49 months ) ; 10 patients were lost to follow-up .
	manualset3
106813	3	402706	5	NULL	NULL	0	NULL	10 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean follow-up was 24.4 months ( range : 6-49 months ) ; 10 patients were lost to follow-up .
	manualset3
106814	4	402706	5	NULL	NULL	0	NULL	follow-up	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean follow-up was 24.4 months ( range : 6-49 months ) ; 10 patients were lost to follow-up .
	manualset3
106815	5	402706	5	NULL	NULL	0	NULL	Mean follow-up	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean follow-up was 24.4 months ( range : 6-49 months ) ; 10 patients were lost to follow-up .
	manualset3
106816	1	402707	5	NULL	NULL	0	NULL	Mean gaps	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean gaps after 1 , 000 load-unload cycles to a 3.9-N pulp pinch did not approach the clinically important limit of 3 mm in all groups .
	manualset3
106817	2	402707	5	NULL	NULL	0	NULL	1 , 000 load-unload cycles	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean gaps after 1 , 000 load-unload cycles to a 3.9-N pulp pinch did not approach the clinically important limit of 3 mm in all groups .
	manualset3
106818	4	402707	5	NULL	NULL	0	NULL	pulp pinch	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean gaps after 1 , 000 load-unload cycles to a 3.9-N pulp pinch did not approach the clinically important limit of 3 mm in all groups .
	manualset3
106819	3	402707	5	NULL	NULL	0	NULL	3.9-N	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean gaps after 1 , 000 load-unload cycles to a 3.9-N pulp pinch did not approach the clinically important limit of 3 mm in all groups .
	manualset3
106820	5	402707	5	NULL	NULL	0	NULL	clinically important limit	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean gaps after 1 , 000 load-unload cycles to a 3.9-N pulp pinch did not approach the clinically important limit of 3 mm in all groups .
	manualset3
106821	6	402707	5	NULL	NULL	0	NULL	3 mm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean gaps after 1 , 000 load-unload cycles to a 3.9-N pulp pinch did not approach the clinically important limit of 3 mm in all groups .
	manualset3
106822	7	402707	5	NULL	NULL	0	NULL	groups 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean gaps after 1 , 000 load-unload cycles to a 3.9-N pulp pinch did not approach the clinically important limit of 3 mm in all groups .
	manualset3
106823	1	402708	5	NULL	NULL	0	NULL	benign diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A benign diagnosis can be made in multihormonal euploid tumors weighing less than 200 g. In larger neoplasms and in cases lacking sustentacular cells and showing increased mitotic activity , an unfavourable prognosis is to be suspected and the same therapeutic procedures should be applied as for tumors in which malignancy is evident in metastatic growth .
	manualset3
106824	2	402708	5	NULL	NULL	0	NULL	multihormonal euploid tumors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A benign diagnosis can be made in multihormonal euploid tumors weighing less than 200 g. In larger neoplasms and in cases lacking sustentacular cells and showing increased mitotic activity , an unfavourable prognosis is to be suspected and the same therapeutic procedures should be applied as for tumors in which malignancy is evident in metastatic growth .
	manualset3
106825	3	402708	5	NULL	NULL	0	NULL	200 g	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A benign diagnosis can be made in multihormonal euploid tumors weighing less than 200 g. In larger neoplasms and in cases lacking sustentacular cells and showing increased mitotic activity , an unfavourable prognosis is to be suspected and the same therapeutic procedures should be applied as for tumors in which malignancy is evident in metastatic growth .
	manualset3
106826	4	402708	5	NULL	NULL	0	NULL	larger neoplasms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A benign diagnosis can be made in multihormonal euploid tumors weighing less than 200 g. In larger neoplasms and in cases lacking sustentacular cells and showing increased mitotic activity , an unfavourable prognosis is to be suspected and the same therapeutic procedures should be applied as for tumors in which malignancy is evident in metastatic growth .
	manualset3
106827	5	402708	5	NULL	NULL	0	NULL	sustentacular cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A benign diagnosis can be made in multihormonal euploid tumors weighing less than 200 g. In larger neoplasms and in cases lacking sustentacular cells and showing increased mitotic activity , an unfavourable prognosis is to be suspected and the same therapeutic procedures should be applied as for tumors in which malignancy is evident in metastatic growth .
	manualset3
106828	6	402708	5	NULL	NULL	NULL	NULL	mitotic activity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A benign diagnosis can be made in multihormonal euploid tumors weighing less than 200 g. In larger neoplasms and in cases lacking sustentacular cells and showing increased mitotic activity , an unfavourable prognosis is to be suspected and the same therapeutic procedures should be applied as for tumors in which malignancy is evident in metastatic growth .
	manualset3
106829	7	402708	5	NULL	NULL	0	NULL	unfavourable prognosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A benign diagnosis can be made in multihormonal euploid tumors weighing less than 200 g. In larger neoplasms and in cases lacking sustentacular cells and showing increased mitotic activity , an unfavourable prognosis is to be suspected and the same therapeutic procedures should be applied as for tumors in which malignancy is evident in metastatic growth .
	manualset3
106830	8	402708	5	NULL	NULL	0	NULL	therapeutic procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A benign diagnosis can be made in multihormonal euploid tumors weighing less than 200 g. In larger neoplasms and in cases lacking sustentacular cells and showing increased mitotic activity , an unfavourable prognosis is to be suspected and the same therapeutic procedures should be applied as for tumors in which malignancy is evident in metastatic growth .
	manualset3
106831	9	402708	5	NULL	NULL	0	NULL	tumors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A benign diagnosis can be made in multihormonal euploid tumors weighing less than 200 g. In larger neoplasms and in cases lacking sustentacular cells and showing increased mitotic activity , an unfavourable prognosis is to be suspected and the same therapeutic procedures should be applied as for tumors in which malignancy is evident in metastatic growth .
	manualset3
106832	10	402708	5	NULL	NULL	0	NULL	malignancy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A benign diagnosis can be made in multihormonal euploid tumors weighing less than 200 g. In larger neoplasms and in cases lacking sustentacular cells and showing increased mitotic activity , an unfavourable prognosis is to be suspected and the same therapeutic procedures should be applied as for tumors in which malignancy is evident in metastatic growth .
	manualset3
106833	11	402708	5	NULL	NULL	0	NULL	metastatic growth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A benign diagnosis can be made in multihormonal euploid tumors weighing less than 200 g. In larger neoplasms and in cases lacking sustentacular cells and showing increased mitotic activity , an unfavourable prognosis is to be suspected and the same therapeutic procedures should be applied as for tumors in which malignancy is evident in metastatic growth .
	manualset3
106834	1	402709	5	NULL	NULL	0	NULL	Mean semen zidovudine levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean semen zidovudine levels ( as measured by a new radioimmunoassay ) in samples collected 0.75 to 1.25 hours after oral dosing were 3.63 to 7.19 mumol/L .
	manualset3
106835	2	402709	5	NULL	NULL	0	NULL	new radioimmunoassay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean semen zidovudine levels ( as measured by a new radioimmunoassay ) in samples collected 0.75 to 1.25 hours after oral dosing were 3.63 to 7.19 mumol/L .
	manualset3
106836	3	402709	5	NULL	NULL	0	NULL	samples 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean semen zidovudine levels ( as measured by a new radioimmunoassay ) in samples collected 0.75 to 1.25 hours after oral dosing were 3.63 to 7.19 mumol/L .
	manualset3
106837	4	402709	5	NULL	NULL	0	NULL	0.75 to 1.25 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean semen zidovudine levels ( as measured by a new radioimmunoassay ) in samples collected 0.75 to 1.25 hours after oral dosing were 3.63 to 7.19 mumol/L .
	manualset3
106838	5	402709	5	NULL	NULL	0	NULL	oral dosing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean semen zidovudine levels ( as measured by a new radioimmunoassay ) in samples collected 0.75 to 1.25 hours after oral dosing were 3.63 to 7.19 mumol/L .
	manualset3
112972	6	402709	5	NULL	NULL	0	NULL	3.63 to 7.19 mumol/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean semen zidovudine levels ( as measured by a new radioimmunoassay ) in samples collected 0.75 to 1.25 hours after oral dosing were 3.63 to 7.19 mumol/L .
	manualset3
106839	1	402710	5	NULL	NULL	0	NULL	Mean stimulation index ( SI )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean stimulation index ( SI ) in response to solubilized TSH receptor was significantly increased only in hyperthyroid GD patients ( SI = 3.0 + / - 1.8 SD , n = 13 , p less than 0.025 ) when compared to normal subjects ( SI = 1.5 + / - 0.8 SD , n = 14 ) .
	manualset3
106840	2	402710	5	NULL	NULL	0	NULL	response 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean stimulation index ( SI ) in response to solubilized TSH receptor was significantly increased only in hyperthyroid GD patients ( SI = 3.0 + / - 1.8 SD , n = 13 , p less than 0.025 ) when compared to normal subjects ( SI = 1.5 + / - 0.8 SD , n = 14 ) .
	manualset3
106841	3	402710	5	NULL	NULL	0	NULL	solubilized TSH receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean stimulation index ( SI ) in response to solubilized TSH receptor was significantly increased only in hyperthyroid GD patients ( SI = 3.0 + / - 1.8 SD , n = 13 , p less than 0.025 ) when compared to normal subjects ( SI = 1.5 + / - 0.8 SD , n = 14 ) .
	manualset3
106842	4	402710	5	NULL	NULL	0	NULL	hyperthyroid GD patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean stimulation index ( SI ) in response to solubilized TSH receptor was significantly increased only in hyperthyroid GD patients ( SI = 3.0 + / - 1.8 SD , n = 13 , p less than 0.025 ) when compared to normal subjects ( SI = 1.5 + / - 0.8 SD , n = 14 ) .
	manualset3
106843	5	402710	5	NULL	NULL	0	NULL	SI = 3.0 + / - 1.8 SD 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean stimulation index ( SI ) in response to solubilized TSH receptor was significantly increased only in hyperthyroid GD patients ( SI = 3.0 + / - 1.8 SD , n = 13 , p less than 0.025 ) when compared to normal subjects ( SI = 1.5 + / - 0.8 SD , n = 14 ) .
	manualset3
106844	6	402710	5	NULL	NULL	0	NULL	n = 13 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean stimulation index ( SI ) in response to solubilized TSH receptor was significantly increased only in hyperthyroid GD patients ( SI = 3.0 + / - 1.8 SD , n = 13 , p less than 0.025 ) when compared to normal subjects ( SI = 1.5 + / - 0.8 SD , n = 14 ) .
	manualset3
106845	7	402710	5	NULL	NULL	0	NULL	p less than 0.025	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean stimulation index ( SI ) in response to solubilized TSH receptor was significantly increased only in hyperthyroid GD patients ( SI = 3.0 + / - 1.8 SD , n = 13 , p less than 0.025 ) when compared to normal subjects ( SI = 1.5 + / - 0.8 SD , n = 14 ) .
	manualset3
106846	8	402710	5	NULL	NULL	0	NULL	normal subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean stimulation index ( SI ) in response to solubilized TSH receptor was significantly increased only in hyperthyroid GD patients ( SI = 3.0 + / - 1.8 SD , n = 13 , p less than 0.025 ) when compared to normal subjects ( SI = 1.5 + / - 0.8 SD , n = 14 ) .
	manualset3
106847	9	402710	5	NULL	NULL	0	NULL	SI = 1.5 + / - 0.8 SD	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean stimulation index ( SI ) in response to solubilized TSH receptor was significantly increased only in hyperthyroid GD patients ( SI = 3.0 + / - 1.8 SD , n = 13 , p less than 0.025 ) when compared to normal subjects ( SI = 1.5 + / - 0.8 SD , n = 14 ) .
	manualset3
106848	10	402710	5	NULL	NULL	0	NULL	n = 14	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean stimulation index ( SI ) in response to solubilized TSH receptor was significantly increased only in hyperthyroid GD patients ( SI = 3.0 + / - 1.8 SD , n = 13 , p less than 0.025 ) when compared to normal subjects ( SI = 1.5 + / - 0.8 SD , n = 14 ) .
	manualset3
106849	1	402711	5	NULL	NULL	0	NULL	Mean values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean values of metabolic clearance and secretion rates of GH in steers were 21 liters/h and 252 micrograms/h or 74.5 ml/kg/h and 0.91 microgram/kg/h , respectively .
	manualset3
106850	2	402711	5	NULL	NULL	0	NULL	metabolic clearance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean values of metabolic clearance and secretion rates of GH in steers were 21 liters/h and 252 micrograms/h or 74.5 ml/kg/h and 0.91 microgram/kg/h , respectively .
	manualset3
106851	3	402711	5	NULL	NULL	0	NULL	secretion rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean values of metabolic clearance and secretion rates of GH in steers were 21 liters/h and 252 micrograms/h or 74.5 ml/kg/h and 0.91 microgram/kg/h , respectively .
	manualset3
106852	4	402711	5	NULL	NULL	0	NULL	GH 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean values of metabolic clearance and secretion rates of GH in steers were 21 liters/h and 252 micrograms/h or 74.5 ml/kg/h and 0.91 microgram/kg/h , respectively .
	manualset3
106853	5	402711	5	NULL	NULL	0	NULL	steers	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean values of metabolic clearance and secretion rates of GH in steers were 21 liters/h and 252 micrograms/h or 74.5 ml/kg/h and 0.91 microgram/kg/h , respectively .
	manualset3
106854	6	402711	5	NULL	NULL	0	NULL	21 liters/h 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean values of metabolic clearance and secretion rates of GH in steers were 21 liters/h and 252 micrograms/h or 74.5 ml/kg/h and 0.91 microgram/kg/h , respectively .
	manualset3
106855	7	402711	5	NULL	NULL	0	NULL	252 micrograms/h	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean values of metabolic clearance and secretion rates of GH in steers were 21 liters/h and 252 micrograms/h or 74.5 ml/kg/h and 0.91 microgram/kg/h , respectively .
	manualset3
106856	8	402711	5	NULL	NULL	0	NULL	74.5 ml/kg/h 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean values of metabolic clearance and secretion rates of GH in steers were 21 liters/h and 252 micrograms/h or 74.5 ml/kg/h and 0.91 microgram/kg/h , respectively .
	manualset3
106857	9	402711	5	NULL	NULL	0	NULL	0.91 microgram/kg/h	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean values of metabolic clearance and secretion rates of GH in steers were 21 liters/h and 252 micrograms/h or 74.5 ml/kg/h and 0.91 microgram/kg/h , respectively .
	manualset3
106858	1	402712	5	NULL	NULL	0	NULL	response 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Meanwhile , the response of the V4 cell under study was tested by flashing behaviorally irrelevant bar stimuli in the cell 's classical receptive field ( CRF ) .
	manualset3
106859	2	402712	5	NULL	NULL	0	NULL	V4 cell 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Meanwhile , the response of the V4 cell under study was tested by flashing behaviorally irrelevant bar stimuli in the cell 's classical receptive field ( CRF ) .
	manualset3
106860	3	402712	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Meanwhile , the response of the V4 cell under study was tested by flashing behaviorally irrelevant bar stimuli in the cell 's classical receptive field ( CRF ) .
	manualset3
106861	4	402712	5	NULL	NULL	0	NULL	behaviorally irrelevant bar stimuli	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Meanwhile , the response of the V4 cell under study was tested by flashing behaviorally irrelevant bar stimuli in the cell 's classical receptive field ( CRF ) .
	manualset3
106862	5	402712	5	NULL	NULL	0	NULL	cell 's classical receptive field ( CRF )	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Meanwhile , the response of the V4 cell under study was tested by flashing behaviorally irrelevant bar stimuli in the cell 's classical receptive field ( CRF ) .
	manualset3
106863	1	402713	5	NULL	NULL	0	NULL	work 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Meanwhile , this work identified that ALAS2 is a novel target gene for p300/CBP action as histone acetyltransferases .
	manualset3
106864	2	402713	5	NULL	NULL	0	NULL	 ALAS2	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Meanwhile , this work identified that ALAS2 is a novel target gene for p300/CBP action as histone acetyltransferases .
	manualset3
106865	3	402713	5	NULL	NULL	0	NULL	novel target gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Meanwhile , this work identified that ALAS2 is a novel target gene for p300/CBP action as histone acetyltransferases .
	manualset3
106866	4	402713	5	NULL	NULL	0	NULL	p300/CBP action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Meanwhile , this work identified that ALAS2 is a novel target gene for p300/CBP action as histone acetyltransferases .
	manualset3
106867	5	402713	5	NULL	NULL	0	NULL	histone acetyltransferases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Meanwhile , this work identified that ALAS2 is a novel target gene for p300/CBP action as histone acetyltransferases .
	manualset3
106868	1	402714	5	NULL	NULL	NULL	NULL	Measles vaccine responses	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Measles vaccine responses vary between individuals , and poor immunogenicity is likely to preclude protection against measles .
	manualset3
106869	2	402714	5	NULL	NULL	0	NULL	individuals 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Measles vaccine responses vary between individuals , and poor immunogenicity is likely to preclude protection against measles .
	manualset3
106870	3	402714	5	NULL	NULL	NULL	NULL	poor immunogenicity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Measles vaccine responses vary between individuals , and poor immunogenicity is likely to preclude protection against measles .
	manualset3
106871	4	402714	5	NULL	NULL	NULL	NULL	protection 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Measles vaccine responses vary between individuals , and poor immunogenicity is likely to preclude protection against measles .
	manualset3
106872	5	402714	5	NULL	NULL	0	NULL	measles 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Measles vaccine responses vary between individuals , and poor immunogenicity is likely to preclude protection against measles .
	manualset3
106873	1	402715	5	NULL	NULL	0	NULL	acute systemic toxicity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurable acute systemic toxicity has been low .
	manualset3
106874	1	402716	5	NULL	NULL	0	NULL	air-filled porosities	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Measured air-filled porosities were accurately predicted from measurements of bulk density , moisture , and organic matter content .
	manualset3
106875	2	402716	5	NULL	NULL	0	NULL	measurements 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measured air-filled porosities were accurately predicted from measurements of bulk density , moisture , and organic matter content .
	manualset3
106876	3	402716	5	NULL	NULL	0	NULL	bulk density	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Measured air-filled porosities were accurately predicted from measurements of bulk density , moisture , and organic matter content .
	manualset3
106877	4	402716	5	NULL	NULL	0	NULL	moisture 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Measured air-filled porosities were accurately predicted from measurements of bulk density , moisture , and organic matter content .
	manualset3
106878	5	402716	5	NULL	NULL	0	NULL	organic matter content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measured air-filled porosities were accurately predicted from measurements of bulk density , moisture , and organic matter content .
	manualset3
106879	1	402717	5	NULL	NULL	0	NULL	internal concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measured internal concentrations of carbazole , dibenzothiophene , and acridine increased with increasing soil concentrations , but biota-soil accumulation factors were low ( 0.002-0 .1 ) .
	manualset3
106880	2	402717	5	NULL	NULL	0	NULL	carbazole 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Measured internal concentrations of carbazole , dibenzothiophene , and acridine increased with increasing soil concentrations , but biota-soil accumulation factors were low ( 0.002-0 .1 ) .
	manualset3
106881	3	402717	5	NULL	NULL	0	NULL	dibenzothiophene 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Measured internal concentrations of carbazole , dibenzothiophene , and acridine increased with increasing soil concentrations , but biota-soil accumulation factors were low ( 0.002-0 .1 ) .
	manualset3
106882	4	402717	5	NULL	NULL	0	NULL	acridine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Measured internal concentrations of carbazole , dibenzothiophene , and acridine increased with increasing soil concentrations , but biota-soil accumulation factors were low ( 0.002-0 .1 ) .
	manualset3
106883	5	402717	5	NULL	NULL	0	NULL	soil concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measured internal concentrations of carbazole , dibenzothiophene , and acridine increased with increasing soil concentrations , but biota-soil accumulation factors were low ( 0.002-0 .1 ) .
	manualset3
106884	6	402717	5	NULL	NULL	0	NULL	biota-soil accumulation factors	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Measured internal concentrations of carbazole , dibenzothiophene , and acridine increased with increasing soil concentrations , but biota-soil accumulation factors were low ( 0.002-0 .1 ) .
	manualset3
106885	7	402717	5	NULL	NULL	0	NULL	0.002-0 .1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Measured internal concentrations of carbazole , dibenzothiophene , and acridine increased with increasing soil concentrations , but biota-soil accumulation factors were low ( 0.002-0 .1 ) .
	manualset3
106886	1	402718	5	NULL	NULL	0	NULL	Measured oxygen consumption	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measured oxygen consumption correlated with Qtd ( r = .78 ) nearly as well as did Qc , while mixed venous oxygen saturation correlated poorly with Qtd ( r = -.10 ) .
	manualset3
106887	2	402718	5	NULL	NULL	0	NULL	Qtd	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measured oxygen consumption correlated with Qtd ( r = .78 ) nearly as well as did Qc , while mixed venous oxygen saturation correlated poorly with Qtd ( r = -.10 ) .
	manualset3
106888	3	402718	5	NULL	NULL	0	NULL	r = .78 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Measured oxygen consumption correlated with Qtd ( r = .78 ) nearly as well as did Qc , while mixed venous oxygen saturation correlated poorly with Qtd ( r = -.10 ) .
	manualset3
106889	4	402718	5	NULL	NULL	0	NULL	Qc	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measured oxygen consumption correlated with Qtd ( r = .78 ) nearly as well as did Qc , while mixed venous oxygen saturation correlated poorly with Qtd ( r = -.10 ) .
	manualset3
106890	5	402718	5	NULL	NULL	0	NULL	mixed venous oxygen saturation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measured oxygen consumption correlated with Qtd ( r = .78 ) nearly as well as did Qc , while mixed venous oxygen saturation correlated poorly with Qtd ( r = -.10 ) .
	manualset3
106891	6	402718	5	NULL	NULL	0	NULL	Qtd 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measured oxygen consumption correlated with Qtd ( r = .78 ) nearly as well as did Qc , while mixed venous oxygen saturation correlated poorly with Qtd ( r = -.10 ) .
	manualset3
106892	7	402718	5	NULL	NULL	0	NULL	 r = -.10	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Measured oxygen consumption correlated with Qtd ( r = .78 ) nearly as well as did Qc , while mixed venous oxygen saturation correlated poorly with Qtd ( r = -.10 ) .
	manualset3
106893	2	402719	5	NULL	NULL	NULL	NULL	APRT activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Measurement of APRT activity showed a complete dificiency in this patient ( less than 0.02 % ) .
	manualset3
106894	1	402719	5	NULL	NULL	0	NULL	Measurement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of APRT activity showed a complete dificiency in this patient ( less than 0.02 % ) .
	manualset3
106895	3	402719	5	NULL	NULL	0	NULL	complete dificiency 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of APRT activity showed a complete dificiency in this patient ( less than 0.02 % ) .
	manualset3
106896	4	402719	5	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of APRT activity showed a complete dificiency in this patient ( less than 0.02 % ) .
	manualset3
106897	5	402719	5	NULL	NULL	0	NULL	less than 0.02 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of APRT activity showed a complete dificiency in this patient ( less than 0.02 % ) .
	manualset3
106898	1	402720	5	NULL	NULL	0	NULL	Measurement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of CPT by a neurometer is a useful tool to evaluate the neurotoxicity of anticancer drugs objectively .
	manualset3
106899	2	402720	5	NULL	NULL	0	NULL	CPT 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of CPT by a neurometer is a useful tool to evaluate the neurotoxicity of anticancer drugs objectively .
	manualset3
106900	3	402720	5	NULL	NULL	0	NULL	neurometer 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of CPT by a neurometer is a useful tool to evaluate the neurotoxicity of anticancer drugs objectively .
	manualset3
106901	4	402720	5	NULL	NULL	0	NULL	useful tool	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of CPT by a neurometer is a useful tool to evaluate the neurotoxicity of anticancer drugs objectively .
	manualset3
106902	5	402720	5	NULL	NULL	0	NULL	neurotoxicity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of CPT by a neurometer is a useful tool to evaluate the neurotoxicity of anticancer drugs objectively .
	manualset3
106903	6	402720	5	NULL	NULL	0	NULL	 anticancer drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of CPT by a neurometer is a useful tool to evaluate the neurotoxicity of anticancer drugs objectively .
	manualset3
106904	1	402721	5	NULL	NULL	0	NULL	better method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A better method for standardizing vitellogenin content of fish tissues .
	manualset3
106905	2	402721	5	NULL	NULL	0	NULL	vitellogenin content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A better method for standardizing vitellogenin content of fish tissues .
	manualset3
106906	3	402721	5	NULL	NULL	0	NULL	fish tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	A better method for standardizing vitellogenin content of fish tissues .
	manualset3
106907	1	402722	5	NULL	NULL	0	NULL	Measurement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of blood morphine concentrations in the victims showed no significant difference from the concentrations noted in a control group of heroin addicts dying from causes other than overdosage .
	manualset3
106908	2	402722	5	NULL	NULL	0	NULL	blood morphine concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of blood morphine concentrations in the victims showed no significant difference from the concentrations noted in a control group of heroin addicts dying from causes other than overdosage .
	manualset3
106909	3	402722	5	NULL	NULL	0	NULL	victims 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of blood morphine concentrations in the victims showed no significant difference from the concentrations noted in a control group of heroin addicts dying from causes other than overdosage .
	manualset3
106910	4	402722	5	NULL	NULL	0	NULL	concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of blood morphine concentrations in the victims showed no significant difference from the concentrations noted in a control group of heroin addicts dying from causes other than overdosage .
	manualset3
106911	5	402722	5	NULL	NULL	0	NULL	control group of heroin addicts 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of blood morphine concentrations in the victims showed no significant difference from the concentrations noted in a control group of heroin addicts dying from causes other than overdosage .
	manualset3
106912	6	402722	5	NULL	NULL	0	NULL	overdosage 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of blood morphine concentrations in the victims showed no significant difference from the concentrations noted in a control group of heroin addicts dying from causes other than overdosage .
	manualset3
106913	1	402723	5	NULL	NULL	0	NULL	Measurement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of gastric acid secretion in the rat by test meal : effects of distension , pentagastrin and propantheline .
	manualset3
106914	2	402723	5	NULL	NULL	0	NULL	gastric acid secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of gastric acid secretion in the rat by test meal : effects of distension , pentagastrin and propantheline .
	manualset3
106915	3	402723	5	NULL	NULL	0	NULL	rat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of gastric acid secretion in the rat by test meal : effects of distension , pentagastrin and propantheline .
	manualset3
106916	4	402723	5	NULL	NULL	0	NULL	test meal	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of gastric acid secretion in the rat by test meal : effects of distension , pentagastrin and propantheline .
	manualset3
106917	5	402723	5	NULL	NULL	0	NULL	distension 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of gastric acid secretion in the rat by test meal : effects of distension , pentagastrin and propantheline .
	manualset3
106918	6	402723	5	NULL	NULL	0	NULL	pentagastrin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of gastric acid secretion in the rat by test meal : effects of distension , pentagastrin and propantheline .
	manualset3
106919	7	402723	5	NULL	NULL	0	NULL	propantheline 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of gastric acid secretion in the rat by test meal : effects of distension , pentagastrin and propantheline .
	manualset3
106920	1	402724	5	NULL	NULL	0	NULL	Measurement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of the metabolic interconversion of deuterium-labeled fatty acids by gas chromatography/mass spectrometry .
	manualset3
106921	2	402724	5	NULL	NULL	0	NULL	metabolic interconversion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of the metabolic interconversion of deuterium-labeled fatty acids by gas chromatography/mass spectrometry .
	manualset3
106922	3	402724	5	NULL	NULL	0	NULL	deuterium-labeled fatty acids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of the metabolic interconversion of deuterium-labeled fatty acids by gas chromatography/mass spectrometry .
	manualset3
106923	4	402724	5	NULL	NULL	0	NULL	gas chromatography/mass spectrometry 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of the metabolic interconversion of deuterium-labeled fatty acids by gas chromatography/mass spectrometry .
	manualset3
106924	1	402725	5	NULL	NULL	0	NULL	Measurements 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements in PRP after stimulation with collagen showed a significant decrease in PDGF ( from 21.5 + / - 1.4 pg / ( mL x 10 ( 6 ) platelets ) to 1.8 + / - 4.1 ( pg/mL x 10 ( 6 ) platelets ) , in beta-TG ( from 21.0 + / - 13.3 ng / ( mL x 10 ( 6 ) platelets ) to 2.2 + / - 1.4 ng / ( mL x 10 ( 6 ) platelets ) ) and in TxB2 ( from 143.6 + / - 80.7 pg / ( mL x 10 ( 6 ) platelets ) to 0.5 + / - 0.6 pg / ( mL x 10 ( 6 ) platelets ) ) after treatment with ASA .
	manualset3
106925	2	402725	5	NULL	NULL	0	NULL	PRP 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements in PRP after stimulation with collagen showed a significant decrease in PDGF ( from 21.5 + / - 1.4 pg / ( mL x 10 ( 6 ) platelets ) to 1.8 + / - 4.1 ( pg/mL x 10 ( 6 ) platelets ) , in beta-TG ( from 21.0 + / - 13.3 ng / ( mL x 10 ( 6 ) platelets ) to 2.2 + / - 1.4 ng / ( mL x 10 ( 6 ) platelets ) ) and in TxB2 ( from 143.6 + / - 80.7 pg / ( mL x 10 ( 6 ) platelets ) to 0.5 + / - 0.6 pg / ( mL x 10 ( 6 ) platelets ) ) after treatment with ASA .
	manualset3
106926	3	402725	5	NULL	NULL	0	NULL	stimulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements in PRP after stimulation with collagen showed a significant decrease in PDGF ( from 21.5 + / - 1.4 pg / ( mL x 10 ( 6 ) platelets ) to 1.8 + / - 4.1 ( pg/mL x 10 ( 6 ) platelets ) , in beta-TG ( from 21.0 + / - 13.3 ng / ( mL x 10 ( 6 ) platelets ) to 2.2 + / - 1.4 ng / ( mL x 10 ( 6 ) platelets ) ) and in TxB2 ( from 143.6 + / - 80.7 pg / ( mL x 10 ( 6 ) platelets ) to 0.5 + / - 0.6 pg / ( mL x 10 ( 6 ) platelets ) ) after treatment with ASA .
	manualset3
106927	4	402725	5	NULL	NULL	0	NULL	collagen 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements in PRP after stimulation with collagen showed a significant decrease in PDGF ( from 21.5 + / - 1.4 pg / ( mL x 10 ( 6 ) platelets ) to 1.8 + / - 4.1 ( pg/mL x 10 ( 6 ) platelets ) , in beta-TG ( from 21.0 + / - 13.3 ng / ( mL x 10 ( 6 ) platelets ) to 2.2 + / - 1.4 ng / ( mL x 10 ( 6 ) platelets ) ) and in TxB2 ( from 143.6 + / - 80.7 pg / ( mL x 10 ( 6 ) platelets ) to 0.5 + / - 0.6 pg / ( mL x 10 ( 6 ) platelets ) ) after treatment with ASA .
	manualset3
106928	5	402725	5	NULL	NULL	0	NULL	PDGF 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements in PRP after stimulation with collagen showed a significant decrease in PDGF ( from 21.5 + / - 1.4 pg / ( mL x 10 ( 6 ) platelets ) to 1.8 + / - 4.1 ( pg/mL x 10 ( 6 ) platelets ) , in beta-TG ( from 21.0 + / - 13.3 ng / ( mL x 10 ( 6 ) platelets ) to 2.2 + / - 1.4 ng / ( mL x 10 ( 6 ) platelets ) ) and in TxB2 ( from 143.6 + / - 80.7 pg / ( mL x 10 ( 6 ) platelets ) to 0.5 + / - 0.6 pg / ( mL x 10 ( 6 ) platelets ) ) after treatment with ASA .
	manualset3
106929	6	402725	5	NULL	NULL	0	NULL	21.5 + / - 1.4 pg / ( mL x 10 ( 6 ) platelets	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements in PRP after stimulation with collagen showed a significant decrease in PDGF ( from 21.5 + / - 1.4 pg / ( mL x 10 ( 6 ) platelets ) to 1.8 + / - 4.1 ( pg/mL x 10 ( 6 ) platelets ) , in beta-TG ( from 21.0 + / - 13.3 ng / ( mL x 10 ( 6 ) platelets ) to 2.2 + / - 1.4 ng / ( mL x 10 ( 6 ) platelets ) ) and in TxB2 ( from 143.6 + / - 80.7 pg / ( mL x 10 ( 6 ) platelets ) to 0.5 + / - 0.6 pg / ( mL x 10 ( 6 ) platelets ) ) after treatment with ASA .
	manualset3
106930	7	402725	5	NULL	NULL	0	NULL	1.8 + / - 4.1 ( pg/mL x 10 ( 6 ) platelets )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements in PRP after stimulation with collagen showed a significant decrease in PDGF ( from 21.5 + / - 1.4 pg / ( mL x 10 ( 6 ) platelets ) to 1.8 + / - 4.1 ( pg/mL x 10 ( 6 ) platelets ) , in beta-TG ( from 21.0 + / - 13.3 ng / ( mL x 10 ( 6 ) platelets ) to 2.2 + / - 1.4 ng / ( mL x 10 ( 6 ) platelets ) ) and in TxB2 ( from 143.6 + / - 80.7 pg / ( mL x 10 ( 6 ) platelets ) to 0.5 + / - 0.6 pg / ( mL x 10 ( 6 ) platelets ) ) after treatment with ASA .
	manualset3
106931	8	402725	5	NULL	NULL	0	NULL	beta-TG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements in PRP after stimulation with collagen showed a significant decrease in PDGF ( from 21.5 + / - 1.4 pg / ( mL x 10 ( 6 ) platelets ) to 1.8 + / - 4.1 ( pg/mL x 10 ( 6 ) platelets ) , in beta-TG ( from 21.0 + / - 13.3 ng / ( mL x 10 ( 6 ) platelets ) to 2.2 + / - 1.4 ng / ( mL x 10 ( 6 ) platelets ) ) and in TxB2 ( from 143.6 + / - 80.7 pg / ( mL x 10 ( 6 ) platelets ) to 0.5 + / - 0.6 pg / ( mL x 10 ( 6 ) platelets ) ) after treatment with ASA .
	manualset3
106932	9	402725	5	NULL	NULL	0	NULL	21.0 + / - 13.3 ng / ( mL x 10 ( 6 ) platelets 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements in PRP after stimulation with collagen showed a significant decrease in PDGF ( from 21.5 + / - 1.4 pg / ( mL x 10 ( 6 ) platelets ) to 1.8 + / - 4.1 ( pg/mL x 10 ( 6 ) platelets ) , in beta-TG ( from 21.0 + / - 13.3 ng / ( mL x 10 ( 6 ) platelets ) to 2.2 + / - 1.4 ng / ( mL x 10 ( 6 ) platelets ) ) and in TxB2 ( from 143.6 + / - 80.7 pg / ( mL x 10 ( 6 ) platelets ) to 0.5 + / - 0.6 pg / ( mL x 10 ( 6 ) platelets ) ) after treatment with ASA .
	manualset3
106933	10	402725	5	NULL	NULL	0	NULL	2.2 + / - 1.4 ng / ( mL x 10 ( 6 ) platelets ) )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements in PRP after stimulation with collagen showed a significant decrease in PDGF ( from 21.5 + / - 1.4 pg / ( mL x 10 ( 6 ) platelets ) to 1.8 + / - 4.1 ( pg/mL x 10 ( 6 ) platelets ) , in beta-TG ( from 21.0 + / - 13.3 ng / ( mL x 10 ( 6 ) platelets ) to 2.2 + / - 1.4 ng / ( mL x 10 ( 6 ) platelets ) ) and in TxB2 ( from 143.6 + / - 80.7 pg / ( mL x 10 ( 6 ) platelets ) to 0.5 + / - 0.6 pg / ( mL x 10 ( 6 ) platelets ) ) after treatment with ASA .
	manualset3
106934	11	402725	5	NULL	NULL	0	NULL	TxB2 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements in PRP after stimulation with collagen showed a significant decrease in PDGF ( from 21.5 + / - 1.4 pg / ( mL x 10 ( 6 ) platelets ) to 1.8 + / - 4.1 ( pg/mL x 10 ( 6 ) platelets ) , in beta-TG ( from 21.0 + / - 13.3 ng / ( mL x 10 ( 6 ) platelets ) to 2.2 + / - 1.4 ng / ( mL x 10 ( 6 ) platelets ) ) and in TxB2 ( from 143.6 + / - 80.7 pg / ( mL x 10 ( 6 ) platelets ) to 0.5 + / - 0.6 pg / ( mL x 10 ( 6 ) platelets ) ) after treatment with ASA .
	manualset3
106935	12	402725	5	NULL	NULL	0	NULL	143.6 + / - 80.7 pg / ( mL x 10 ( 6 ) platelets )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements in PRP after stimulation with collagen showed a significant decrease in PDGF ( from 21.5 + / - 1.4 pg / ( mL x 10 ( 6 ) platelets ) to 1.8 + / - 4.1 ( pg/mL x 10 ( 6 ) platelets ) , in beta-TG ( from 21.0 + / - 13.3 ng / ( mL x 10 ( 6 ) platelets ) to 2.2 + / - 1.4 ng / ( mL x 10 ( 6 ) platelets ) ) and in TxB2 ( from 143.6 + / - 80.7 pg / ( mL x 10 ( 6 ) platelets ) to 0.5 + / - 0.6 pg / ( mL x 10 ( 6 ) platelets ) ) after treatment with ASA .
	manualset3
106936	13	402725	5	NULL	NULL	0	NULL	143.6 + / - 80.7 pg / ( mL x 10 ( 6 ) platelets )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements in PRP after stimulation with collagen showed a significant decrease in PDGF ( from 21.5 + / - 1.4 pg / ( mL x 10 ( 6 ) platelets ) to 1.8 + / - 4.1 ( pg/mL x 10 ( 6 ) platelets ) , in beta-TG ( from 21.0 + / - 13.3 ng / ( mL x 10 ( 6 ) platelets ) to 2.2 + / - 1.4 ng / ( mL x 10 ( 6 ) platelets ) ) and in TxB2 ( from 143.6 + / - 80.7 pg / ( mL x 10 ( 6 ) platelets ) to 0.5 + / - 0.6 pg / ( mL x 10 ( 6 ) platelets ) ) after treatment with ASA .
	manualset3
106937	14	402725	5	NULL	NULL	0	NULL	0.5 + / - 0.6 pg / ( mL x 10 ( 6 ) platelets ) )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements in PRP after stimulation with collagen showed a significant decrease in PDGF ( from 21.5 + / - 1.4 pg / ( mL x 10 ( 6 ) platelets ) to 1.8 + / - 4.1 ( pg/mL x 10 ( 6 ) platelets ) , in beta-TG ( from 21.0 + / - 13.3 ng / ( mL x 10 ( 6 ) platelets ) to 2.2 + / - 1.4 ng / ( mL x 10 ( 6 ) platelets ) ) and in TxB2 ( from 143.6 + / - 80.7 pg / ( mL x 10 ( 6 ) platelets ) to 0.5 + / - 0.6 pg / ( mL x 10 ( 6 ) platelets ) ) after treatment with ASA .
	manualset3
106938	15	402725	5	NULL	NULL	0	NULL	treatment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements in PRP after stimulation with collagen showed a significant decrease in PDGF ( from 21.5 + / - 1.4 pg / ( mL x 10 ( 6 ) platelets ) to 1.8 + / - 4.1 ( pg/mL x 10 ( 6 ) platelets ) , in beta-TG ( from 21.0 + / - 13.3 ng / ( mL x 10 ( 6 ) platelets ) to 2.2 + / - 1.4 ng / ( mL x 10 ( 6 ) platelets ) ) and in TxB2 ( from 143.6 + / - 80.7 pg / ( mL x 10 ( 6 ) platelets ) to 0.5 + / - 0.6 pg / ( mL x 10 ( 6 ) platelets ) ) after treatment with ASA .
	manualset3
106939	16	402725	5	NULL	NULL	0	NULL	ASA 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements in PRP after stimulation with collagen showed a significant decrease in PDGF ( from 21.5 + / - 1.4 pg / ( mL x 10 ( 6 ) platelets ) to 1.8 + / - 4.1 ( pg/mL x 10 ( 6 ) platelets ) , in beta-TG ( from 21.0 + / - 13.3 ng / ( mL x 10 ( 6 ) platelets ) to 2.2 + / - 1.4 ng / ( mL x 10 ( 6 ) platelets ) ) and in TxB2 ( from 143.6 + / - 80.7 pg / ( mL x 10 ( 6 ) platelets ) to 0.5 + / - 0.6 pg / ( mL x 10 ( 6 ) platelets ) ) after treatment with ASA .
	manualset3
106940	1	402726	5	NULL	NULL	0	NULL	Measurements 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements of CP-violating asymmetries in B0 -- ) a1 + / - ( 1260 ) pi - / + decays .
	manualset3
106941	2	402726	5	NULL	NULL	0	NULL	CP-violating asymmetries	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements of CP-violating asymmetries in B0 -- ) a1 + / - ( 1260 ) pi - / + decays .
	manualset3
106942	3	402726	5	NULL	NULL	0	NULL	B0 -- ) a1 + / - ( 1260 ) pi - / + decays	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements of CP-violating asymmetries in B0 -- ) a1 + / - ( 1260 ) pi - / + decays .
	manualset3
106943	1	402727	5	NULL	NULL	0	NULL	Measurements 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements of furosemide concentrations in the urine , however , confirmed that sufficient amounts were applied to inhibit the feedback mechanism .
	manualset3
106944	2	402727	5	NULL	NULL	0	NULL	furosemide concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements of furosemide concentrations in the urine , however , confirmed that sufficient amounts were applied to inhibit the feedback mechanism .
	manualset3
106945	3	402727	5	NULL	NULL	0	NULL	urine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements of furosemide concentrations in the urine , however , confirmed that sufficient amounts were applied to inhibit the feedback mechanism .
	manualset3
106946	4	402727	5	NULL	NULL	0	NULL	sufficient amounts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements of furosemide concentrations in the urine , however , confirmed that sufficient amounts were applied to inhibit the feedback mechanism .
	manualset3
106947	5	402727	5	NULL	NULL	0	NULL	inhibit 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements of furosemide concentrations in the urine , however , confirmed that sufficient amounts were applied to inhibit the feedback mechanism .
	manualset3
106948	6	402727	5	NULL	NULL	0	NULL	feedback mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements of furosemide concentrations in the urine , however , confirmed that sufficient amounts were applied to inhibit the feedback mechanism .
	manualset3
106949	1	402728	5	NULL	NULL	0	NULL	Measurements 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements of intravascular pressures and volumes often fail to predict the response to fluids , even though very low values are usually associated with a positive response to fluids .
	manualset3
106950	2	402728	5	NULL	NULL	0	NULL	intravascular pressures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements of intravascular pressures and volumes often fail to predict the response to fluids , even though very low values are usually associated with a positive response to fluids .
	manualset3
106951	3	402728	5	NULL	NULL	0	NULL	volumes 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements of intravascular pressures and volumes often fail to predict the response to fluids , even though very low values are usually associated with a positive response to fluids .
	manualset3
106952	4	402728	5	NULL	NULL	0	NULL	response 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements of intravascular pressures and volumes often fail to predict the response to fluids , even though very low values are usually associated with a positive response to fluids .
	manualset3
106953	5	402728	5	NULL	NULL	0	NULL	fluids 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements of intravascular pressures and volumes often fail to predict the response to fluids , even though very low values are usually associated with a positive response to fluids .
	manualset3
106954	6	402728	5	NULL	NULL	0	NULL	very low values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements of intravascular pressures and volumes often fail to predict the response to fluids , even though very low values are usually associated with a positive response to fluids .
	manualset3
106955	7	402728	5	NULL	NULL	0	NULL	positive response	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements of intravascular pressures and volumes often fail to predict the response to fluids , even though very low values are usually associated with a positive response to fluids .
	manualset3
106956	8	402728	5	NULL	NULL	0	NULL	fluids 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements of intravascular pressures and volumes often fail to predict the response to fluids , even though very low values are usually associated with a positive response to fluids .
	manualset3
106957	1	402729	5	NULL	NULL	0	NULL	Measurements 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements of nanoparticle dissolution at both low and high pH show that zinc ions can be released into the aqueous phase and that humic acid under certain , but not all , conditions can increase Zn ( 2 + ) ( aq ) concentrations .
	manualset3
106958	2	402729	5	NULL	NULL	0	NULL	nanoparticle dissolution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements of nanoparticle dissolution at both low and high pH show that zinc ions can be released into the aqueous phase and that humic acid under certain , but not all , conditions can increase Zn ( 2 + ) ( aq ) concentrations .
	manualset3
106959	3	402729	5	NULL	NULL	0	NULL	low pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements of nanoparticle dissolution at both low and high pH show that zinc ions can be released into the aqueous phase and that humic acid under certain , but not all , conditions can increase Zn ( 2 + ) ( aq ) concentrations .
	manualset3
106960	4	402729	5	NULL	NULL	NULL	NULL	high pH	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Measurements of nanoparticle dissolution at both low and high pH show that zinc ions can be released into the aqueous phase and that humic acid under certain , but not all , conditions can increase Zn ( 2 + ) ( aq ) concentrations .
	manualset3
106961	5	402729	5	NULL	NULL	0	NULL	zinc ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements of nanoparticle dissolution at both low and high pH show that zinc ions can be released into the aqueous phase and that humic acid under certain , but not all , conditions can increase Zn ( 2 + ) ( aq ) concentrations .
	manualset3
106962	6	402729	5	NULL	NULL	0	NULL	aqueous phase 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements of nanoparticle dissolution at both low and high pH show that zinc ions can be released into the aqueous phase and that humic acid under certain , but not all , conditions can increase Zn ( 2 + ) ( aq ) concentrations .
	manualset3
106963	7	402729	5	NULL	NULL	0	NULL	humic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements of nanoparticle dissolution at both low and high pH show that zinc ions can be released into the aqueous phase and that humic acid under certain , but not all , conditions can increase Zn ( 2 + ) ( aq ) concentrations .
	manualset3
106964	8	402729	5	NULL	NULL	0	NULL	conditions 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements of nanoparticle dissolution at both low and high pH show that zinc ions can be released into the aqueous phase and that humic acid under certain , but not all , conditions can increase Zn ( 2 + ) ( aq ) concentrations .
	manualset3
112973	9	402729	5	NULL	NULL	NULL	NULL	Zn ( 2 + ) ( aq ) concentrations	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Measurements of nanoparticle dissolution at both low and high pH show that zinc ions can be released into the aqueous phase and that humic acid under certain , but not all , conditions can increase Zn ( 2 + ) ( aq ) concentrations .
	manualset3
106965	1	402730	5	NULL	NULL	0	NULL	bi-directional transient displacement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A bi-directional transient displacement of cytoplasm is observed during expansion and collapse of the cavitation bubble .
	manualset3
106966	2	402730	5	NULL	NULL	0	NULL	cytoplasm 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A bi-directional transient displacement of cytoplasm is observed during expansion and collapse of the cavitation bubble .
	manualset3
106967	3	402730	5	NULL	NULL	0	NULL	expansion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A bi-directional transient displacement of cytoplasm is observed during expansion and collapse of the cavitation bubble .
	manualset3
106968	4	402730	5	NULL	NULL	0	NULL	collapse 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A bi-directional transient displacement of cytoplasm is observed during expansion and collapse of the cavitation bubble .
	manualset3
106969	5	402730	5	NULL	NULL	0	NULL	cavitation bubble	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A bi-directional transient displacement of cytoplasm is observed during expansion and collapse of the cavitation bubble .
	manualset3
106970	1	402731	5	NULL	NULL	0	NULL	Measurements 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements of radon around closed uranium mines .
	manualset3
106971	2	402731	5	NULL	NULL	0	NULL	radon 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements of radon around closed uranium mines .
	manualset3
106972	3	402731	5	NULL	NULL	0	NULL	uranium mines	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements of radon around closed uranium mines .
	manualset3
106973	1	402732	5	NULL	NULL	0	NULL	Measurements 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements were conducted at temperatures of 326 , 339 , 352 and 363K .
	manualset3
106974	2	402732	5	NULL	NULL	0	NULL	temperatures 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements were conducted at temperatures of 326 , 339 , 352 and 363K .
	manualset3
106975	3	402732	5	NULL	NULL	0	NULL	326 K	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements were conducted at temperatures of 326 , 339 , 352 and 363K .
	manualset3
106976	4	402732	5	NULL	NULL	0	NULL	339 K	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements were conducted at temperatures of 326 , 339 , 352 and 363K .
	manualset3
106977	5	402732	5	NULL	NULL	0	NULL	352 K	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements were conducted at temperatures of 326 , 339 , 352 and 363K .
	manualset3
106978	5	402732	5	NULL	NULL	0	NULL	352 K	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements were conducted at temperatures of 326 , 339 , 352 and 363K .
	manualset3
106979	6	402732	5	NULL	NULL	0	NULL	363K	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements were conducted at temperatures of 326 , 339 , 352 and 363K .
	manualset3
106980	1	402733	5	NULL	NULL	0	NULL	Measurements 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements were performed for one basal state and for five subcritical incremental stenoses created with a screw occluder during hyperemia .
	manualset3
106981	2	402733	5	NULL	NULL	NULL	NULL	basal state	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Measurements were performed for one basal state and for five subcritical incremental stenoses created with a screw occluder during hyperemia .
	manualset3
106982	3	402733	5	NULL	NULL	0	NULL	five subcritical incremental stenoses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements were performed for one basal state and for five subcritical incremental stenoses created with a screw occluder during hyperemia .
	manualset3
106983	4	402733	5	NULL	NULL	0	NULL	screw occluder	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements were performed for one basal state and for five subcritical incremental stenoses created with a screw occluder during hyperemia .
	manualset3
106984	5	402733	5	NULL	NULL	0	NULL	hyperemia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements were performed for one basal state and for five subcritical incremental stenoses created with a screw occluder during hyperemia .
	manualset3
106985	1	402734	5	NULL	NULL	0	NULL	inhalation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measures to prevent the inhalation of papain dust must be taken in factories where papain is handled , not only to avoid the proteolytic effects of the material but also to prevent workers from becoming sensitised .
	manualset3
106986	2	402734	5	NULL	NULL	0	NULL	papain dust 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Measures to prevent the inhalation of papain dust must be taken in factories where papain is handled , not only to avoid the proteolytic effects of the material but also to prevent workers from becoming sensitised .
	manualset3
106987	3	402734	5	NULL	NULL	0	NULL	factories 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Measures to prevent the inhalation of papain dust must be taken in factories where papain is handled , not only to avoid the proteolytic effects of the material but also to prevent workers from becoming sensitised .
	manualset3
106988	4	402734	5	NULL	NULL	0	NULL	papain 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Measures to prevent the inhalation of papain dust must be taken in factories where papain is handled , not only to avoid the proteolytic effects of the material but also to prevent workers from becoming sensitised .
	manualset3
106989	5	402734	5	NULL	NULL	0	NULL	proteolytic effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measures to prevent the inhalation of papain dust must be taken in factories where papain is handled , not only to avoid the proteolytic effects of the material but also to prevent workers from becoming sensitised .
	manualset3
106990	6	402734	5	NULL	NULL	0	NULL	material 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measures to prevent the inhalation of papain dust must be taken in factories where papain is handled , not only to avoid the proteolytic effects of the material but also to prevent workers from becoming sensitised .
	manualset3
106991	7	402734	5	NULL	NULL	NULL	NULL	workers	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Measures to prevent the inhalation of papain dust must be taken in factories where papain is handled , not only to avoid the proteolytic effects of the material but also to prevent workers from becoming sensitised .
	manualset3
106992	1	402735	5	NULL	NULL	0	NULL	participation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measuring participation in childhood disability : how does the capability approach improve our understanding ?
	manualset3
106993	2	402735	5	NULL	NULL	0	NULL	childhood disability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Measuring participation in childhood disability : how does the capability approach improve our understanding ?
	manualset3
106994	3	402735	5	NULL	NULL	0	NULL	capability approach	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Measuring participation in childhood disability : how does the capability approach improve our understanding ?
	manualset3
106995	4	402735	5	NULL	NULL	0	NULL	understanding 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Measuring participation in childhood disability : how does the capability approach improve our understanding ?
	manualset3
106996	1	402736	5	NULL	NULL	0	NULL	quality 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measuring quality of pharmacotherapy for depression in a national health care system .
	manualset3
106997	2	402736	5	NULL	NULL	0	NULL	pharmacotherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Measuring quality of pharmacotherapy for depression in a national health care system .
	manualset3
106998	3	402736	5	NULL	NULL	0	NULL	depression 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Measuring quality of pharmacotherapy for depression in a national health care system .
	manualset3
106999	4	402736	5	NULL	NULL	0	NULL	national health care system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Measuring quality of pharmacotherapy for depression in a national health care system .
	manualset3
107000	1	402737	5	NULL	NULL	0	NULL	Mechanical activities 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanical activities of the uterus , cervix , and bladder were recorded in vivo in anesthetized rats during electrical stimulation of either the hypogastric or pelvic nerve .
	manualset3
107001	2	402737	5	NULL	NULL	0	NULL	uterus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanical activities of the uterus , cervix , and bladder were recorded in vivo in anesthetized rats during electrical stimulation of either the hypogastric or pelvic nerve .
	manualset3
107002	3	402737	5	NULL	NULL	0	NULL	cervix 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanical activities of the uterus , cervix , and bladder were recorded in vivo in anesthetized rats during electrical stimulation of either the hypogastric or pelvic nerve .
	manualset3
107003	4	402737	5	NULL	NULL	0	NULL	bladder 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanical activities of the uterus , cervix , and bladder were recorded in vivo in anesthetized rats during electrical stimulation of either the hypogastric or pelvic nerve .
	manualset3
107004	5	402737	5	NULL	NULL	0	NULL	anesthetized rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanical activities of the uterus , cervix , and bladder were recorded in vivo in anesthetized rats during electrical stimulation of either the hypogastric or pelvic nerve .
	manualset3
107005	6	402737	5	NULL	NULL	0	NULL	electrical stimulation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanical activities of the uterus , cervix , and bladder were recorded in vivo in anesthetized rats during electrical stimulation of either the hypogastric or pelvic nerve .
	manualset3
107006	7	402737	5	NULL	NULL	0	NULL	hypogastric nerve	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanical activities of the uterus , cervix , and bladder were recorded in vivo in anesthetized rats during electrical stimulation of either the hypogastric or pelvic nerve .
	manualset3
107007	8	402737	5	NULL	NULL	0	NULL	pelvic nerve	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanical activities of the uterus , cervix , and bladder were recorded in vivo in anesthetized rats during electrical stimulation of either the hypogastric or pelvic nerve .
	manualset3
107081	1	402738	5	NULL	NULL	0	NULL	Mechanical characteristics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanical characteristics of cross-stitch epitenon suture in association with various two-strand core sutures : a biomechanical study using canine cadaver tendons .
	manualset3
107082	2	402738	5	NULL	NULL	0	NULL	cross-stitch epitenon suture	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanical characteristics of cross-stitch epitenon suture in association with various two-strand core sutures : a biomechanical study using canine cadaver tendons .
	manualset3
107083	3	402738	5	NULL	NULL	0	NULL	association 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanical characteristics of cross-stitch epitenon suture in association with various two-strand core sutures : a biomechanical study using canine cadaver tendons .
	manualset3
107092	4	402738	5	NULL	NULL	0	NULL	two-strand core sutures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanical characteristics of cross-stitch epitenon suture in association with various two-strand core sutures : a biomechanical study using canine cadaver tendons .
	manualset3
107093	5	402738	5	NULL	NULL	0	NULL	biomechanical study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanical characteristics of cross-stitch epitenon suture in association with various two-strand core sutures : a biomechanical study using canine cadaver tendons .
	manualset3
107094	6	402738	5	NULL	NULL	0	NULL	canine cadaver tendons	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanical characteristics of cross-stitch epitenon suture in association with various two-strand core sutures : a biomechanical study using canine cadaver tendons .
	manualset3
107095	1	402739	5	NULL	NULL	NULL	NULL	bifunctional spiro-type organocatalyst	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A bifunctional spiro-type organocatalyst with high enantiocontrol : application to the aza-Morita-Baylis-Hillman reactions .
	manualset3
107096	2	402739	5	NULL	NULL	0	NULL	enantiocontrol 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A bifunctional spiro-type organocatalyst with high enantiocontrol : application to the aza-Morita-Baylis-Hillman reactions .
	manualset3
107106	3	402739	5	NULL	NULL	0	NULL	application 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A bifunctional spiro-type organocatalyst with high enantiocontrol : application to the aza-Morita-Baylis-Hillman reactions .
	manualset3
107107	4	402739	5	NULL	NULL	0	NULL	aza-Morita-Baylis-Hillman reactions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A bifunctional spiro-type organocatalyst with high enantiocontrol : application to the aza-Morita-Baylis-Hillman reactions .
	manualset3
107118	1	402740	5	NULL	NULL	0	NULL	Mechanical impedance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanical impedance of the femur : a preliminary report .
	manualset3
107120	2	402740	5	NULL	NULL	0	NULL	femur 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanical impedance of the femur : a preliminary report .
	manualset3
107121	3	402740	5	NULL	NULL	0	NULL	preliminary report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanical impedance of the femur : a preliminary report .
	manualset3
107122	1	402741	5	NULL	NULL	0	NULL	Mechanical stimulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanical stimulation of skin organ cultures from HR-1 , nNOS-KO , endothelial NOS-KO ( eNOS-KO ) , and WT mice caused an enlargement of cutaneous lymphatic vessels .
	manualset3
107124	2	402741	5	NULL	NULL	0	NULL	skin organ cultures	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanical stimulation of skin organ cultures from HR-1 , nNOS-KO , endothelial NOS-KO ( eNOS-KO ) , and WT mice caused an enlargement of cutaneous lymphatic vessels .
	manualset3
107135	3	402741	5	NULL	NULL	0	NULL	HR-1 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanical stimulation of skin organ cultures from HR-1 , nNOS-KO , endothelial NOS-KO ( eNOS-KO ) , and WT mice caused an enlargement of cutaneous lymphatic vessels .
	manualset3
107137	4	402741	5	NULL	NULL	0	NULL	nNOS-KO mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanical stimulation of skin organ cultures from HR-1 , nNOS-KO , endothelial NOS-KO ( eNOS-KO ) , and WT mice caused an enlargement of cutaneous lymphatic vessels .
	manualset3
107139	5	402741	5	NULL	NULL	0	NULL	endothelial NOS-KO ( eNOS-KO ) mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanical stimulation of skin organ cultures from HR-1 , nNOS-KO , endothelial NOS-KO ( eNOS-KO ) , and WT mice caused an enlargement of cutaneous lymphatic vessels .
	manualset3
107140	6	402741	5	NULL	NULL	0	NULL	WT mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanical stimulation of skin organ cultures from HR-1 , nNOS-KO , endothelial NOS-KO ( eNOS-KO ) , and WT mice caused an enlargement of cutaneous lymphatic vessels .
	manualset3
107143	7	402741	5	NULL	NULL	0	NULL	enlargement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanical stimulation of skin organ cultures from HR-1 , nNOS-KO , endothelial NOS-KO ( eNOS-KO ) , and WT mice caused an enlargement of cutaneous lymphatic vessels .
	manualset3
107145	8	402741	5	NULL	NULL	0	NULL	cutaneous lymphatic vessels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanical stimulation of skin organ cultures from HR-1 , nNOS-KO , endothelial NOS-KO ( eNOS-KO ) , and WT mice caused an enlargement of cutaneous lymphatic vessels .
	manualset3
107164	1	402742	5	NULL	NULL	0	NULL	Mechanical unfolding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanical unfolding of RNA hairpins .
	manualset3
107165	2	402742	5	NULL	NULL	0	NULL	RNA hairpins	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanical unfolding of RNA hairpins .
	manualset3
107167	1	402743	5	NULL	NULL	0	NULL	Mechanically adaptive intracortical implants	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanically adaptive intracortical implants improve the proximity of neuronal cell bodies .
	manualset3
107169	2	402743	5	NULL	NULL	0	NULL	proximity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanically adaptive intracortical implants improve the proximity of neuronal cell bodies .
	manualset3
107171	3	402743	5	NULL	NULL	NULL	NULL	neuronal cell bodies	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mechanically adaptive intracortical implants improve the proximity of neuronal cell bodies .
	manualset3
107174	1	402744	5	NULL	NULL	0	NULL	Mechanism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism and control of pyrrole synthesis .
	manualset3
107176	2	402744	5	NULL	NULL	0	NULL	control 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism and control of pyrrole synthesis .
	manualset3
107179	3	402744	5	NULL	NULL	0	NULL	pyrrole synthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism and control of pyrrole synthesis .
	manualset3
107180	1	402745	5	NULL	NULL	0	NULL	Mechanism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of Cu ( A ) assembly .
	manualset3
107181	2	402745	5	NULL	NULL	0	NULL	Cu ( A ) assembly	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of Cu ( A ) assembly .
	manualset3
107182	1	402746	5	NULL	NULL	0	NULL	Mechanism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of action of a new antialdosterone compound , prorenone .
	manualset3
107184	2	402746	5	NULL	NULL	0	NULL	action 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of action of a new antialdosterone compound , prorenone .
	manualset3
107188	3	402746	5	NULL	NULL	0	NULL	antialdosterone compound	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of action of a new antialdosterone compound , prorenone .
	manualset3
107189	4	402746	5	NULL	NULL	0	NULL	prorenone 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of action of a new antialdosterone compound , prorenone .
	manualset3
107191	1	402747	5	NULL	NULL	0	NULL	Mechanism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of action of clonazepam in myoclonus in relation to effects on GABA and 5-HT .
	manualset3
107193	2	402747	5	NULL	NULL	0	NULL	action 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of action of clonazepam in myoclonus in relation to effects on GABA and 5-HT .
	manualset3
107194	3	402747	5	NULL	NULL	0	NULL	clonazepam 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of action of clonazepam in myoclonus in relation to effects on GABA and 5-HT .
	manualset3
107199	4	402747	5	NULL	NULL	0	NULL	myoclonus 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of action of clonazepam in myoclonus in relation to effects on GABA and 5-HT .
	manualset3
107200	5	402747	5	NULL	NULL	0	NULL	relation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of action of clonazepam in myoclonus in relation to effects on GABA and 5-HT .
	manualset3
107201	6	402747	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of action of clonazepam in myoclonus in relation to effects on GABA and 5-HT .
	manualset3
107202	7	402747	5	NULL	NULL	0	NULL	GABA 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of action of clonazepam in myoclonus in relation to effects on GABA and 5-HT .
	manualset3
107203	8	402747	5	NULL	NULL	0	NULL	5-HT	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of action of clonazepam in myoclonus in relation to effects on GABA and 5-HT .
	manualset3
107204	1	402748	5	NULL	NULL	0	NULL	bimodal particle dynamics model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A bimodal particle dynamics model considering coagulation , coalescence and surface growth , and its application to the growth of titania aggregates .
	manualset3
107205	2	402748	5	NULL	NULL	0	NULL	coagulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A bimodal particle dynamics model considering coagulation , coalescence and surface growth , and its application to the growth of titania aggregates .
	manualset3
107206	3	402748	5	NULL	NULL	0	NULL	coalescence 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A bimodal particle dynamics model considering coagulation , coalescence and surface growth , and its application to the growth of titania aggregates .
	manualset3
107208	4	402748	5	NULL	NULL	0	NULL	surface growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A bimodal particle dynamics model considering coagulation , coalescence and surface growth , and its application to the growth of titania aggregates .
	manualset3
107210	5	402748	5	NULL	NULL	0	NULL	application 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A bimodal particle dynamics model considering coagulation , coalescence and surface growth , and its application to the growth of titania aggregates .
	manualset3
107212	6	402748	5	NULL	NULL	0	NULL	growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A bimodal particle dynamics model considering coagulation , coalescence and surface growth , and its application to the growth of titania aggregates .
	manualset3
107214	7	402748	5	NULL	NULL	0	NULL	titania aggregates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A bimodal particle dynamics model considering coagulation , coalescence and surface growth , and its application to the growth of titania aggregates .
	manualset3
107215	1	402749	5	NULL	NULL	0	NULL	Mechanism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of action of the antiviral compound MDL 20 , 610 .
	manualset3
107217	2	402749	5	NULL	NULL	0	NULL	action 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of action of the antiviral compound MDL 20 , 610 .
	manualset3
107220	3	402749	5	NULL	NULL	0	NULL	antiviral compound MDL 20 , 610	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of action of the antiviral compound MDL 20 , 610 .
	manualset3
107221	1	402750	5	NULL	NULL	0	NULL	Mechanism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of action of type II , glycoengineered , anti-CD20 monoclonal antibody GA101 in B-chronic lymphocytic leukemia whole blood assays in comparison with rituximab and alemtuzumab .
	manualset3
107222	2	402750	5	NULL	NULL	0	NULL	action 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of action of type II , glycoengineered , anti-CD20 monoclonal antibody GA101 in B-chronic lymphocytic leukemia whole blood assays in comparison with rituximab and alemtuzumab .
	manualset3
107223	3	402750	5	NULL	NULL	0	NULL	type II, glycoengineered, anti-CD20 monoclonal antibody GA101	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of action of type II , glycoengineered , anti-CD20 monoclonal antibody GA101 in B-chronic lymphocytic leukemia whole blood assays in comparison with rituximab and alemtuzumab .
	manualset3
107224	4	402750	5	NULL	NULL	0	NULL	B-chronic lymphocytic leukemia whole blood assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of action of type II , glycoengineered , anti-CD20 monoclonal antibody GA101 in B-chronic lymphocytic leukemia whole blood assays in comparison with rituximab and alemtuzumab .
	manualset3
107225	5	402750	5	NULL	NULL	0	NULL	comparison 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of action of type II , glycoengineered , anti-CD20 monoclonal antibody GA101 in B-chronic lymphocytic leukemia whole blood assays in comparison with rituximab and alemtuzumab .
	manualset3
107226	6	402750	5	NULL	NULL	0	NULL	rituximab 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of action of type II , glycoengineered , anti-CD20 monoclonal antibody GA101 in B-chronic lymphocytic leukemia whole blood assays in comparison with rituximab and alemtuzumab .
	manualset3
107227	7	402750	5	NULL	NULL	0	NULL	alemtuzumab 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of action of type II , glycoengineered , anti-CD20 monoclonal antibody GA101 in B-chronic lymphocytic leukemia whole blood assays in comparison with rituximab and alemtuzumab .
	manualset3
107228	1	402751	5	NULL	NULL	0	NULL	Mechanism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of chemiluminescence from the linoleate -- lipoxygenase system .
	manualset3
107229	2	402751	5	NULL	NULL	0	NULL	chemiluminescence 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of chemiluminescence from the linoleate -- lipoxygenase system .
	manualset3
107230	3	402751	5	NULL	NULL	0	NULL	linoleate -- lipoxygenase system	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of chemiluminescence from the linoleate -- lipoxygenase system .
	manualset3
107231	1	402752	5	NULL	NULL	0	NULL	Mechanism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of glucose-6-phosphate dehydrogenase-mediated regulation of coronary artery contractility .
	manualset3
107232	2	402752	5	NULL	NULL	0	NULL	glucose-6-phosphate dehydrogenase-mediated regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of glucose-6-phosphate dehydrogenase-mediated regulation of coronary artery contractility .
	manualset3
107233	3	402752	5	NULL	NULL	0	NULL	coronary artery contractility	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of glucose-6-phosphate dehydrogenase-mediated regulation of coronary artery contractility .
	manualset3
107234	1	402753	5	NULL	NULL	0	NULL	Mechanism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of injury was blunt in 198 and penetrating in 14 patients .
	manualset3
107235	2	402753	5	NULL	NULL	0	NULL	injury 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of injury was blunt in 198 and penetrating in 14 patients .
	manualset3
107236	3	402753	5	NULL	NULL	0	NULL	198 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of injury was blunt in 198 and penetrating in 14 patients .
	manualset3
107237	4	402753	5	NULL	NULL	0	NULL	14 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of injury was blunt in 198 and penetrating in 14 patients .
	manualset3
107238	1	402754	5	NULL	NULL	0	NULL	Mechanism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of reversal by deoxycytidine .
	manualset3
107239	2	402754	5	NULL	NULL	0	NULL	reversal 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of reversal by deoxycytidine .
	manualset3
107240	3	402754	5	NULL	NULL	0	NULL	deoxycytidine 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of reversal by deoxycytidine .
	manualset3
107241	1	402755	5	NULL	NULL	0	NULL	Mechanism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of silver particle formation during photoreduction using in situ time-resolved SAXS analysis .
	manualset3
107242	2	402755	5	NULL	NULL	0	NULL	silver particle formation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of silver particle formation during photoreduction using in situ time-resolved SAXS analysis .
	manualset3
107243	3	402755	5	NULL	NULL	0	NULL	photoreduction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of silver particle formation during photoreduction using in situ time-resolved SAXS analysis .
	manualset3
107244	4	402755	5	NULL	NULL	0	NULL	 in situ time-resolved SAXS analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of silver particle formation during photoreduction using in situ time-resolved SAXS analysis .
	manualset3
107245	1	402756	5	NULL	NULL	0	NULL	Mechanism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of transcription factor recruitment by acidic activators .
	manualset3
107246	2	402756	5	NULL	NULL	0	NULL	transcription factor recruitment	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of transcription factor recruitment by acidic activators .
	manualset3
107247	3	402756	5	NULL	NULL	NULL	NULL	acidic activators	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mechanism of transcription factor recruitment by acidic activators .
	manualset3
107255	1	402757	5	NULL	NULL	0	NULL	Mechanism studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism studies indicated that , like kojic acid , APP showed inhibition toward plant polyphenol oxidase and was able to decolor quinones .
	manualset3
107264	2	402757	5	NULL	NULL	0	NULL	kojic acid	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism studies indicated that , like kojic acid , APP showed inhibition toward plant polyphenol oxidase and was able to decolor quinones .
	manualset3
107266	3	402757	5	NULL	NULL	0	NULL	APP 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism studies indicated that , like kojic acid , APP showed inhibition toward plant polyphenol oxidase and was able to decolor quinones .
	manualset3
107267	4	402757	5	NULL	NULL	0	NULL	inhibition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism studies indicated that , like kojic acid , APP showed inhibition toward plant polyphenol oxidase and was able to decolor quinones .
	manualset3
107268	5	402757	5	NULL	NULL	0	NULL	plant polyphenol oxidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism studies indicated that , like kojic acid , APP showed inhibition toward plant polyphenol oxidase and was able to decolor quinones .
	manualset3
107269	6	402757	5	NULL	NULL	0	NULL	quinones 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism studies indicated that , like kojic acid , APP showed inhibition toward plant polyphenol oxidase and was able to decolor quinones .
	manualset3
107271	1	402758	5	NULL	NULL	0	NULL	Mechanisms 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanisms involved in the inhibition of myoblast proliferation and differentiation by myostatin .
	manualset3
107272	2	402758	5	NULL	NULL	0	NULL	inhibition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanisms involved in the inhibition of myoblast proliferation and differentiation by myostatin .
	manualset3
107274	3	402758	5	NULL	NULL	0	NULL	myoblast proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanisms involved in the inhibition of myoblast proliferation and differentiation by myostatin .
	manualset3
107276	4	402758	5	NULL	NULL	0	NULL	myoblast differentiation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanisms involved in the inhibition of myoblast proliferation and differentiation by myostatin .
	manualset3
107277	5	402758	5	NULL	NULL	0	NULL	myostatin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanisms involved in the inhibition of myoblast proliferation and differentiation by myostatin .
	manualset3
107278	1	402759	5	NULL	NULL	0	NULL	biochemical approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A biochemical and immunological approach to the identification of H-Y antigenic proteins secreted from Daudi cells .
	manualset3
107279	2	402759	5	NULL	NULL	0	NULL	immunological approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A biochemical and immunological approach to the identification of H-Y antigenic proteins secreted from Daudi cells .
	manualset3
107280	3	402759	5	NULL	NULL	0	NULL	identification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A biochemical and immunological approach to the identification of H-Y antigenic proteins secreted from Daudi cells .
	manualset3
107281	4	402759	5	NULL	NULL	0	NULL	H-Y antigenic proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A biochemical and immunological approach to the identification of H-Y antigenic proteins secreted from Daudi cells .
	manualset3
107282	5	402759	5	NULL	NULL	0	NULL	Daudi cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A biochemical and immunological approach to the identification of H-Y antigenic proteins secreted from Daudi cells .
	manualset3
107283	1	402760	5	NULL	NULL	0	NULL	Mechanisms 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanisms of acute hepatic toxicity : chloroform , halothane , and glutathione .
	manualset3
107284	2	402760	5	NULL	NULL	0	NULL	acute hepatic toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanisms of acute hepatic toxicity : chloroform , halothane , and glutathione .
	manualset3
107285	3	402760	5	NULL	NULL	0	NULL	chloroform 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanisms of acute hepatic toxicity : chloroform , halothane , and glutathione .
	manualset3
107286	4	402760	5	NULL	NULL	0	NULL	halothane 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanisms of acute hepatic toxicity : chloroform , halothane , and glutathione .
	manualset3
107287	5	402760	5	NULL	NULL	0	NULL	glutathione 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanisms of acute hepatic toxicity : chloroform , halothane , and glutathione .
	manualset3
107288	1	402761	5	NULL	NULL	0	NULL	Mechanisms 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanisms of resistance to cephalosporin and emergence of O25b-ST131 clone harboring CTX-M-27 - lactamase in extraintestinal pathogenic Escherichia coli from dogs and cats in Japan .
	manualset3
107289	2	402761	5	NULL	NULL	0	NULL	resistance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanisms of resistance to cephalosporin and emergence of O25b-ST131 clone harboring CTX-M-27 - lactamase in extraintestinal pathogenic Escherichia coli from dogs and cats in Japan .
	manualset3
107290	3	402761	5	NULL	NULL	0	NULL	cephalosporin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanisms of resistance to cephalosporin and emergence of O25b-ST131 clone harboring CTX-M-27 - lactamase in extraintestinal pathogenic Escherichia coli from dogs and cats in Japan .
	manualset3
107291	4	402761	5	NULL	NULL	0	NULL	emergence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanisms of resistance to cephalosporin and emergence of O25b-ST131 clone harboring CTX-M-27 - lactamase in extraintestinal pathogenic Escherichia coli from dogs and cats in Japan .
	manualset3
107292	5	402761	5	NULL	NULL	0	NULL	O25b-ST131 clone harboring CTX-M-27 - lactamase	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanisms of resistance to cephalosporin and emergence of O25b-ST131 clone harboring CTX-M-27 - lactamase in extraintestinal pathogenic Escherichia coli from dogs and cats in Japan .
	manualset3
107293	6	402761	5	NULL	NULL	0	NULL	extraintestinal pathogenic Escherichia coli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanisms of resistance to cephalosporin and emergence of O25b-ST131 clone harboring CTX-M-27 - lactamase in extraintestinal pathogenic Escherichia coli from dogs and cats in Japan .
	manualset3
107294	7	402761	5	NULL	NULL	0	NULL	dogs 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanisms of resistance to cephalosporin and emergence of O25b-ST131 clone harboring CTX-M-27 - lactamase in extraintestinal pathogenic Escherichia coli from dogs and cats in Japan .
	manualset3
107295	8	402761	5	NULL	NULL	0	NULL	cats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanisms of resistance to cephalosporin and emergence of O25b-ST131 clone harboring CTX-M-27 - lactamase in extraintestinal pathogenic Escherichia coli from dogs and cats in Japan .
	manualset3
107296	9	402761	5	NULL	NULL	0	NULL	Japan 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanisms of resistance to cephalosporin and emergence of O25b-ST131 clone harboring CTX-M-27 - lactamase in extraintestinal pathogenic Escherichia coli from dogs and cats in Japan .
	manualset3
107297	1	402762	5	NULL	NULL	0	NULL	Mechanistic studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanistic studies indicated that in vitro treatment of bone marrow stromal cell cultures with SK & F 105685 upregulated the production of colony stimulating activity ( CSA ) detectable in a rat CFU-GM assay .
	manualset3
107298	2	402762	5	NULL	NULL	0	NULL	in vitro treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanistic studies indicated that in vitro treatment of bone marrow stromal cell cultures with SK & F 105685 upregulated the production of colony stimulating activity ( CSA ) detectable in a rat CFU-GM assay .
	manualset3
107299	3	402762	5	NULL	NULL	0	NULL	bone marrow stromal cell cultures with SK & F 105685	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanistic studies indicated that in vitro treatment of bone marrow stromal cell cultures with SK & F 105685 upregulated the production of colony stimulating activity ( CSA ) detectable in a rat CFU-GM assay .
	manualset3
107300	4	402762	5	NULL	NULL	0	NULL	production 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanistic studies indicated that in vitro treatment of bone marrow stromal cell cultures with SK & F 105685 upregulated the production of colony stimulating activity ( CSA ) detectable in a rat CFU-GM assay .
	manualset3
107301	5	402762	5	NULL	NULL	0	NULL	colony stimulating activity ( CSA ) 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanistic studies indicated that in vitro treatment of bone marrow stromal cell cultures with SK & F 105685 upregulated the production of colony stimulating activity ( CSA ) detectable in a rat CFU-GM assay .
	manualset3
107302	6	402762	5	NULL	NULL	0	NULL	rat CFU-GM assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanistic studies indicated that in vitro treatment of bone marrow stromal cell cultures with SK & F 105685 upregulated the production of colony stimulating activity ( CSA ) detectable in a rat CFU-GM assay .
	manualset3
107303	1	402763	5	NULL	NULL	0	NULL	 IP-10	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanistically , IP-10 blockade impedes the expansion of peripheral Ag-specific T cells and hinders their migration into the pancreas .
	manualset3
107304	2	402763	5	NULL	NULL	0	NULL	expansion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanistically , IP-10 blockade impedes the expansion of peripheral Ag-specific T cells and hinders their migration into the pancreas .
	manualset3
107305	3	402763	5	NULL	NULL	0	NULL	peripheral Ag-specific T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanistically , IP-10 blockade impedes the expansion of peripheral Ag-specific T cells and hinders their migration into the pancreas .
	manualset3
107306	4	402763	5	NULL	NULL	NULL	NULL	migration 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mechanistically , IP-10 blockade impedes the expansion of peripheral Ag-specific T cells and hinders their migration into the pancreas .
	manualset3
107307	5	402763	5	NULL	NULL	0	NULL	pancreas 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanistically , IP-10 blockade impedes the expansion of peripheral Ag-specific T cells and hinders their migration into the pancreas .
	manualset3
107308	1	402764	5	NULL	NULL	0	NULL	proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanistically , these proteins associate with barbed ends of actin filaments and antagonize filament capping by capping protein ( CapZ ) .
	manualset3
107309	2	402764	5	NULL	NULL	0	NULL	barbed ends of actin filaments	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanistically , these proteins associate with barbed ends of actin filaments and antagonize filament capping by capping protein ( CapZ ) .
	manualset3
107310	3	402764	5	NULL	NULL	0	NULL	filament capping	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanistically , these proteins associate with barbed ends of actin filaments and antagonize filament capping by capping protein ( CapZ ) .
	manualset3
107311	4	402764	5	NULL	NULL	0	NULL	capping protein ( CapZ )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanistically , these proteins associate with barbed ends of actin filaments and antagonize filament capping by capping protein ( CapZ ) .
	manualset3
107312	1	402765	5	NULL	NULL	0	NULL	Median factor usage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Median factor usage was 999 IU kg ( -1 ) ( 768-1248 ) .
	manualset3
107313	2	402765	5	NULL	NULL	0	NULL	999 IU kg ( -1 ) ( 768-1248 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Median factor usage was 999 IU kg ( -1 ) ( 768-1248 ) .
	manualset3
107314	1	402766	5	NULL	NULL	0	NULL	Median percent gastric retentions	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Median percent gastric retentions at 90 min after the standard meal were 57.1 % ( range , 34.0-83 .2 % ) in PWS patients and 40.2 % ( range , 27.2-60 .2 % ) in controls ( P = 0.03 ) .
	manualset3
107315	2	402766	5	NULL	NULL	0	NULL	90 min	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Median percent gastric retentions at 90 min after the standard meal were 57.1 % ( range , 34.0-83 .2 % ) in PWS patients and 40.2 % ( range , 27.2-60 .2 % ) in controls ( P = 0.03 ) .
	manualset3
107316	3	402766	5	NULL	NULL	0	NULL	standard meal	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Median percent gastric retentions at 90 min after the standard meal were 57.1 % ( range , 34.0-83 .2 % ) in PWS patients and 40.2 % ( range , 27.2-60 .2 % ) in controls ( P = 0.03 ) .
	manualset3
107317	4	402766	5	NULL	NULL	0	NULL	57.1 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Median percent gastric retentions at 90 min after the standard meal were 57.1 % ( range , 34.0-83 .2 % ) in PWS patients and 40.2 % ( range , 27.2-60 .2 % ) in controls ( P = 0.03 ) .
	manualset3
107318	5	402766	5	NULL	NULL	0	NULL	 range , 34.0-83 .2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Median percent gastric retentions at 90 min after the standard meal were 57.1 % ( range , 34.0-83 .2 % ) in PWS patients and 40.2 % ( range , 27.2-60 .2 % ) in controls ( P = 0.03 ) .
	manualset3
107319	6	402766	5	NULL	NULL	0	NULL	PWS patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Median percent gastric retentions at 90 min after the standard meal were 57.1 % ( range , 34.0-83 .2 % ) in PWS patients and 40.2 % ( range , 27.2-60 .2 % ) in controls ( P = 0.03 ) .
	manualset3
107320	7	402766	5	NULL	NULL	0	NULL	 40.2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Median percent gastric retentions at 90 min after the standard meal were 57.1 % ( range , 34.0-83 .2 % ) in PWS patients and 40.2 % ( range , 27.2-60 .2 % ) in controls ( P = 0.03 ) .
	manualset3
107321	8	402766	5	NULL	NULL	0	NULL	range , 27.2-60 .2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Median percent gastric retentions at 90 min after the standard meal were 57.1 % ( range , 34.0-83 .2 % ) in PWS patients and 40.2 % ( range , 27.2-60 .2 % ) in controls ( P = 0.03 ) .
	manualset3
107322	9	402766	5	NULL	NULL	0	NULL	controls 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Median percent gastric retentions at 90 min after the standard meal were 57.1 % ( range , 34.0-83 .2 % ) in PWS patients and 40.2 % ( range , 27.2-60 .2 % ) in controls ( P = 0.03 ) .
	manualset3
107323	10	402766	5	NULL	NULL	0	NULL	P = 0.03	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Median percent gastric retentions at 90 min after the standard meal were 57.1 % ( range , 34.0-83 .2 % ) in PWS patients and 40.2 % ( range , 27.2-60 .2 % ) in controls ( P = 0.03 ) .
	manualset3
107324	1	402767	5	NULL	NULL	0	NULL	biological role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A biological role for heparin-induced release of plasma SOD is demonstrated for the first time in this investigation .
	manualset3
107325	2	402767	5	NULL	NULL	0	NULL	heparin-induced release 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A biological role for heparin-induced release of plasma SOD is demonstrated for the first time in this investigation .
	manualset3
107326	3	402767	5	NULL	NULL	0	NULL	plasma SOD	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A biological role for heparin-induced release of plasma SOD is demonstrated for the first time in this investigation .
	manualset3
107327	4	402767	5	NULL	NULL	0	NULL	first time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	A biological role for heparin-induced release of plasma SOD is demonstrated for the first time in this investigation .
	manualset3
107328	5	402767	5	NULL	NULL	0	NULL	investigation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A biological role for heparin-induced release of plasma SOD is demonstrated for the first time in this investigation .
	manualset3
107329	1	402768	5	NULL	NULL	0	NULL	Median plasma BC concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Median plasma BC concentrations after 1 y of supplementation increased from 335 nmol/L at entry to 3163 nmol/L .
	manualset3
107330	2	402768	5	NULL	NULL	0	NULL	1 y	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Median plasma BC concentrations after 1 y of supplementation increased from 335 nmol/L at entry to 3163 nmol/L .
	manualset3
107331	3	402768	5	NULL	NULL	0	NULL	supplementation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Median plasma BC concentrations after 1 y of supplementation increased from 335 nmol/L at entry to 3163 nmol/L .
	manualset3
107332	4	402768	5	NULL	NULL	0	NULL	335 nmol/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Median plasma BC concentrations after 1 y of supplementation increased from 335 nmol/L at entry to 3163 nmol/L .
	manualset3
107333	5	402768	5	NULL	NULL	0	NULL	3163 nmol/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Median plasma BC concentrations after 1 y of supplementation increased from 335 nmol/L at entry to 3163 nmol/L .
	manualset3
107334	1	402769	5	NULL	NULL	0	NULL	Median recovery times 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Median recovery times to 85 % of baseline FEV1 were shorter for budesonide/formoterol ( 1 or 2 inhalations : 3.3 and 2.8 min , respectively ) than salmeterol/fluticasone ( 8.9 min ; P & lt ; 0.001 ) and placebo ( ) 30 min ) .
	manualset3
107335	2	402769	5	NULL	NULL	0	NULL	85 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Median recovery times to 85 % of baseline FEV1 were shorter for budesonide/formoterol ( 1 or 2 inhalations : 3.3 and 2.8 min , respectively ) than salmeterol/fluticasone ( 8.9 min ; P & lt ; 0.001 ) and placebo ( ) 30 min ) .
	manualset3
107336	3	402769	5	NULL	NULL	0	NULL	baseline FEV1	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Median recovery times to 85 % of baseline FEV1 were shorter for budesonide/formoterol ( 1 or 2 inhalations : 3.3 and 2.8 min , respectively ) than salmeterol/fluticasone ( 8.9 min ; P & lt ; 0.001 ) and placebo ( ) 30 min ) .
	manualset3
107337	4	402769	5	NULL	NULL	0	NULL	budesonide/formoterol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Median recovery times to 85 % of baseline FEV1 were shorter for budesonide/formoterol ( 1 or 2 inhalations : 3.3 and 2.8 min , respectively ) than salmeterol/fluticasone ( 8.9 min ; P & lt ; 0.001 ) and placebo ( ) 30 min ) .
	manualset3
107338	5	402769	5	NULL	NULL	0	NULL	1 or 2 inhalations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Median recovery times to 85 % of baseline FEV1 were shorter for budesonide/formoterol ( 1 or 2 inhalations : 3.3 and 2.8 min , respectively ) than salmeterol/fluticasone ( 8.9 min ; P & lt ; 0.001 ) and placebo ( ) 30 min ) .
	manualset3
107339	6	402769	5	NULL	NULL	0	NULL	3.3 and 2.8 min 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Median recovery times to 85 % of baseline FEV1 were shorter for budesonide/formoterol ( 1 or 2 inhalations : 3.3 and 2.8 min , respectively ) than salmeterol/fluticasone ( 8.9 min ; P & lt ; 0.001 ) and placebo ( ) 30 min ) .
	manualset3
107340	7	402769	5	NULL	NULL	0	NULL	salmeterol/fluticasone 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Median recovery times to 85 % of baseline FEV1 were shorter for budesonide/formoterol ( 1 or 2 inhalations : 3.3 and 2.8 min , respectively ) than salmeterol/fluticasone ( 8.9 min ; P & lt ; 0.001 ) and placebo ( ) 30 min ) .
	manualset3
107341	8	402769	5	NULL	NULL	0	NULL	8.9 min ; P & lt ; 0.001 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Median recovery times to 85 % of baseline FEV1 were shorter for budesonide/formoterol ( 1 or 2 inhalations : 3.3 and 2.8 min , respectively ) than salmeterol/fluticasone ( 8.9 min ; P & lt ; 0.001 ) and placebo ( ) 30 min ) .
	manualset3
107342	9	402769	5	NULL	NULL	0	NULL	placebo 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Median recovery times to 85 % of baseline FEV1 were shorter for budesonide/formoterol ( 1 or 2 inhalations : 3.3 and 2.8 min , respectively ) than salmeterol/fluticasone ( 8.9 min ; P & lt ; 0.001 ) and placebo ( ) 30 min ) .
	manualset3
107343	10	402769	5	NULL	NULL	0	NULL	30 min	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Median recovery times to 85 % of baseline FEV1 were shorter for budesonide/formoterol ( 1 or 2 inhalations : 3.3 and 2.8 min , respectively ) than salmeterol/fluticasone ( 8.9 min ; P & lt ; 0.001 ) and placebo ( ) 30 min ) .
	manualset3
107344	1	402770	5	NULL	NULL	0	NULL	Median survival	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Median survival , complete remission rate , first remission duration , and the distribution of CNS leukemia were similar in both groups .
	manualset3
107345	2	402770	5	NULL	NULL	0	NULL	complete remission rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Median survival , complete remission rate , first remission duration , and the distribution of CNS leukemia were similar in both groups .
	manualset3
107346	3	402770	5	NULL	NULL	NULL	NULL	first remission duration	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Median survival , complete remission rate , first remission duration , and the distribution of CNS leukemia were similar in both groups .
	manualset3
107347	4	402770	5	NULL	NULL	0	NULL	distribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Median survival , complete remission rate , first remission duration , and the distribution of CNS leukemia were similar in both groups .
	manualset3
107348	5	402770	5	NULL	NULL	0	NULL	CNS leukemia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Median survival , complete remission rate , first remission duration , and the distribution of CNS leukemia were similar in both groups .
	manualset3
107349	6	402770	5	NULL	NULL	0	NULL	both groups	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Median survival , complete remission rate , first remission duration , and the distribution of CNS leukemia were similar in both groups .
	manualset3
107350	1	402771	5	NULL	NULL	0	NULL	Mediational path analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mediational path analyses revealed that polarized thoughts fully accounted for the impact of prejudice on evaluative polarization .
	manualset3
107351	2	402771	5	NULL	NULL	0	NULL	polarized thoughts	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mediational path analyses revealed that polarized thoughts fully accounted for the impact of prejudice on evaluative polarization .
	manualset3
107352	3	402771	5	NULL	NULL	0	NULL	impact 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mediational path analyses revealed that polarized thoughts fully accounted for the impact of prejudice on evaluative polarization .
	manualset3
107353	4	402771	5	NULL	NULL	0	NULL	prejudice 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mediational path analyses revealed that polarized thoughts fully accounted for the impact of prejudice on evaluative polarization .
	manualset3
107354	5	402771	5	NULL	NULL	0	NULL	evaluative polarization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mediational path analyses revealed that polarized thoughts fully accounted for the impact of prejudice on evaluative polarization .
	manualset3
107355	1	402772	5	NULL	NULL	0	NULL	Medical aspects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical and legal aspects of child abuse are then discussed , with special reference to the problem in Ethiopia .
	manualset3
107356	2	402772	5	NULL	NULL	0	NULL	legal aspects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical and legal aspects of child abuse are then discussed , with special reference to the problem in Ethiopia .
	manualset3
107357	3	402772	5	NULL	NULL	0	NULL	child abuse	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical and legal aspects of child abuse are then discussed , with special reference to the problem in Ethiopia .
	manualset3
107358	4	402772	5	NULL	NULL	0	NULL	special reference 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical and legal aspects of child abuse are then discussed , with special reference to the problem in Ethiopia .
	manualset3
107359	5	402772	5	NULL	NULL	0	NULL	problem 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical and legal aspects of child abuse are then discussed , with special reference to the problem in Ethiopia .
	manualset3
107360	6	402772	5	NULL	NULL	0	NULL	Ethiopia 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical and legal aspects of child abuse are then discussed , with special reference to the problem in Ethiopia .
	manualset3
107361	1	402773	5	NULL	NULL	0	NULL	Medical student perceptions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical student perceptions of the value of the history and physical examination .
	manualset3
107362	2	402773	5	NULL	NULL	0	NULL	value 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical student perceptions of the value of the history and physical examination .
	manualset3
107363	3	402773	5	NULL	NULL	0	NULL	history 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical student perceptions of the value of the history and physical examination .
	manualset3
107364	4	402773	5	NULL	NULL	0	NULL	physical examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical student perceptions of the value of the history and physical examination .
	manualset3
107365	1	402774	5	NULL	NULL	0	NULL	Medical treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical treatment with new anticysticercus drugs can be effective , while surgery may be indicated in selected cases .
	manualset3
107366	2	402774	5	NULL	NULL	0	NULL	anticysticercus drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical treatment with new anticysticercus drugs can be effective , while surgery may be indicated in selected cases .
	manualset3
107367	3	402774	5	NULL	NULL	0	NULL	surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical treatment with new anticysticercus drugs can be effective , while surgery may be indicated in selected cases .
	manualset3
107368	4	402774	5	NULL	NULL	0	NULL	selected cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical treatment with new anticysticercus drugs can be effective , while surgery may be indicated in selected cases .
	manualset3
107369	1	402775	5	NULL	NULL	0	NULL	biomathematical model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A biomathematical model was developed to simulate relapse development in patients with chronic myeloid leukemia ( CML ) following bone marrow transplantation ( BMT ) .
	manualset3
107370	2	402775	5	NULL	NULL	0	NULL	simulate 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A biomathematical model was developed to simulate relapse development in patients with chronic myeloid leukemia ( CML ) following bone marrow transplantation ( BMT ) .
	manualset3
107371	3	402775	5	NULL	NULL	0	NULL	relapse development	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A biomathematical model was developed to simulate relapse development in patients with chronic myeloid leukemia ( CML ) following bone marrow transplantation ( BMT ) .
	manualset3
107372	4	402775	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A biomathematical model was developed to simulate relapse development in patients with chronic myeloid leukemia ( CML ) following bone marrow transplantation ( BMT ) .
	manualset3
107373	5	402775	5	NULL	NULL	0	NULL	chronic myeloid leukemia ( CML )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A biomathematical model was developed to simulate relapse development in patients with chronic myeloid leukemia ( CML ) following bone marrow transplantation ( BMT ) .
	manualset3
107374	6	402775	5	NULL	NULL	0	NULL	bone marrow transplantation ( BMT )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A biomathematical model was developed to simulate relapse development in patients with chronic myeloid leukemia ( CML ) following bone marrow transplantation ( BMT ) .
	manualset3
107375	1	402776	5	NULL	NULL	0	NULL	Medical care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical care and patient variables were measured for 123 hypertensive medical clinic patients .
	manualset3
107376	2	402776	5	NULL	NULL	0	NULL	patient variables	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical care and patient variables were measured for 123 hypertensive medical clinic patients .
	manualset3
107377	3	402776	5	NULL	NULL	0	NULL	123 hypertensive medical clinic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical care and patient variables were measured for 123 hypertensive medical clinic patients .
	manualset3
107378	1	402777	5	NULL	NULL	0	NULL	Medical confidentiality 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical confidentiality and HIV infection .
	manualset3
107379	2	402777	5	NULL	NULL	0	NULL	HIV infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical confidentiality and HIV infection .
	manualset3
107380	1	402778	5	NULL	NULL	0	NULL	Medical residents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical residents found the phone call to be worthwhile and gained valuable insight into their own discharge practices as demonstrated by self-reflection and intended change in discharge practices .
	manualset3
107381	2	402778	5	NULL	NULL	0	NULL	phone call	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical residents found the phone call to be worthwhile and gained valuable insight into their own discharge practices as demonstrated by self-reflection and intended change in discharge practices .
	manualset3
107382	3	402778	5	NULL	NULL	NULL	NULL	valuable insight	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Medical residents found the phone call to be worthwhile and gained valuable insight into their own discharge practices as demonstrated by self-reflection and intended change in discharge practices .
	manualset3
107383	4	402778	5	NULL	NULL	0	NULL	discharge practices	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical residents found the phone call to be worthwhile and gained valuable insight into their own discharge practices as demonstrated by self-reflection and intended change in discharge practices .
	manualset3
107384	5	402778	5	NULL	NULL	NULL	NULL	self-reflection	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Medical residents found the phone call to be worthwhile and gained valuable insight into their own discharge practices as demonstrated by self-reflection and intended change in discharge practices .
	manualset3
107385	6	402778	5	NULL	NULL	0	NULL	change 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical residents found the phone call to be worthwhile and gained valuable insight into their own discharge practices as demonstrated by self-reflection and intended change in discharge practices .
	manualset3
107386	7	402778	5	NULL	NULL	0	NULL	discharge practices	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical residents found the phone call to be worthwhile and gained valuable insight into their own discharge practices as demonstrated by self-reflection and intended change in discharge practices .
	manualset3
107387	1	402779	5	NULL	NULL	0	NULL	Medical statistics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical statistics , patronage and the state : the development of the MRC Statistical Unit , 1911-1948 .
	manualset3
107388	2	402779	5	NULL	NULL	0	NULL	patronage 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical statistics , patronage and the state : the development of the MRC Statistical Unit , 1911-1948 .
	manualset3
107389	3	402779	5	NULL	NULL	0	NULL	state 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical statistics , patronage and the state : the development of the MRC Statistical Unit , 1911-1948 .
	manualset3
107392	4	402779	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical statistics , patronage and the state : the development of the MRC Statistical Unit , 1911-1948 .
	manualset3
107393	5	402779	5	NULL	NULL	0	NULL	MRC Statistical Unit	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical statistics , patronage and the state : the development of the MRC Statistical Unit , 1911-1948 .
	manualset3
107394	6	402779	5	NULL	NULL	0	NULL	1911-1948	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical statistics , patronage and the state : the development of the MRC Statistical Unit , 1911-1948 .
	manualset3
107395	1	402780	5	NULL	NULL	0	NULL	Medicare financial status	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Medicare financial status , budget impact , and sustainability -- which concept is which ?
	manualset3
107396	2	402780	5	NULL	NULL	0	NULL	budget impact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Medicare financial status , budget impact , and sustainability -- which concept is which ?
	manualset3
107397	3	402780	5	NULL	NULL	0	NULL	sustainability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Medicare financial status , budget impact , and sustainability -- which concept is which ?
	manualset3
107398	4	402780	5	NULL	NULL	0	NULL	concept 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Medicare financial status , budget impact , and sustainability -- which concept is which ?
	manualset3
107399	1	402781	5	NULL	NULL	0	NULL	bis-trisurea ligand	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A bis-trisurea ligand assembles with the tetraalkylammonium halides to form the flat ` stave ' structures or ` barrels ' that encapsulate multiple R ( 4 ) N ( + ) guests , depending on the size of the halide anion ( Cl ( - ) or Br ( - ) ) and the R ( 4 ) N ( + ) cation .
	manualset3
107400	2	402781	5	NULL	NULL	0	NULL	tetraalkylammonium halides	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A bis-trisurea ligand assembles with the tetraalkylammonium halides to form the flat ` stave ' structures or ` barrels ' that encapsulate multiple R ( 4 ) N ( + ) guests , depending on the size of the halide anion ( Cl ( - ) or Br ( - ) ) and the R ( 4 ) N ( + ) cation .
	manualset3
107401	3	402781	5	NULL	NULL	0	NULL	flat ` stave ' structures or ` barrels ' 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A bis-trisurea ligand assembles with the tetraalkylammonium halides to form the flat ` stave ' structures or ` barrels ' that encapsulate multiple R ( 4 ) N ( + ) guests , depending on the size of the halide anion ( Cl ( - ) or Br ( - ) ) and the R ( 4 ) N ( + ) cation .
	manualset3
107402	4	402781	5	NULL	NULL	0	NULL	multiple R ( 4 ) N ( + ) guests	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	A bis-trisurea ligand assembles with the tetraalkylammonium halides to form the flat ` stave ' structures or ` barrels ' that encapsulate multiple R ( 4 ) N ( + ) guests , depending on the size of the halide anion ( Cl ( - ) or Br ( - ) ) and the R ( 4 ) N ( + ) cation .
	manualset3
107403	5	402781	5	NULL	NULL	0	NULL	size 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A bis-trisurea ligand assembles with the tetraalkylammonium halides to form the flat ` stave ' structures or ` barrels ' that encapsulate multiple R ( 4 ) N ( + ) guests , depending on the size of the halide anion ( Cl ( - ) or Br ( - ) ) and the R ( 4 ) N ( + ) cation .
	manualset3
107404	6	402781	5	NULL	NULL	0	NULL	halide anion 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	A bis-trisurea ligand assembles with the tetraalkylammonium halides to form the flat ` stave ' structures or ` barrels ' that encapsulate multiple R ( 4 ) N ( + ) guests , depending on the size of the halide anion ( Cl ( - ) or Br ( - ) ) and the R ( 4 ) N ( + ) cation .
	manualset3
107405	7	402781	5	NULL	NULL	0	NULL	Cl ( - ) 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	A bis-trisurea ligand assembles with the tetraalkylammonium halides to form the flat ` stave ' structures or ` barrels ' that encapsulate multiple R ( 4 ) N ( + ) guests , depending on the size of the halide anion ( Cl ( - ) or Br ( - ) ) and the R ( 4 ) N ( + ) cation .
	manualset3
107406	8	402781	5	NULL	NULL	0	NULL	Br ( - ) 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	A bis-trisurea ligand assembles with the tetraalkylammonium halides to form the flat ` stave ' structures or ` barrels ' that encapsulate multiple R ( 4 ) N ( + ) guests , depending on the size of the halide anion ( Cl ( - ) or Br ( - ) ) and the R ( 4 ) N ( + ) cation .
	manualset3
107407	9	402781	5	NULL	NULL	0	NULL	R ( 4 ) N ( + ) cation	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	A bis-trisurea ligand assembles with the tetraalkylammonium halides to form the flat ` stave ' structures or ` barrels ' that encapsulate multiple R ( 4 ) N ( + ) guests , depending on the size of the halide anion ( Cl ( - ) or Br ( - ) ) and the R ( 4 ) N ( + ) cation .
	manualset3
107408	1	402782	5	NULL	NULL	0	NULL	Medication errors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Medication errors in the outpatient setting : classification and root cause analysis .
	manualset3
107409	2	402782	5	NULL	NULL	0	NULL	outpatient setting 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Medication errors in the outpatient setting : classification and root cause analysis .
	manualset3
107410	3	402782	5	NULL	NULL	0	NULL	classification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Medication errors in the outpatient setting : classification and root cause analysis .
	manualset3
107411	4	402782	5	NULL	NULL	0	NULL	root cause analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Medication errors in the outpatient setting : classification and root cause analysis .
	manualset3
107412	1	402783	5	NULL	NULL	0	NULL	Medicine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Medicine is being treated as a business , with cost curtailment measures and profit margins often dictating physicians ' choices .
	manualset3
107413	2	402783	5	NULL	NULL	0	NULL	business 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Medicine is being treated as a business , with cost curtailment measures and profit margins often dictating physicians ' choices .
	manualset3
107414	3	402783	5	NULL	NULL	0	NULL	cost curtailment measures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Medicine is being treated as a business , with cost curtailment measures and profit margins often dictating physicians ' choices .
	manualset3
107415	4	402783	5	NULL	NULL	0	NULL	profit margins	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Medicine is being treated as a business , with cost curtailment measures and profit margins often dictating physicians ' choices .
	manualset3
107416	5	402783	5	NULL	NULL	0	NULL	physicians ' choices	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Medicine is being treated as a business , with cost curtailment measures and profit margins often dictating physicians ' choices .
	manualset3
107417	1	402784	5	NULL	NULL	0	NULL	Medium osmolality	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Medium osmolality was altered to simulate hyposmotic ( 190 + / - 10 mmol/kg ) or hyperosmotic conditions ( 400 + / - 10 mmol/kg ) , whereas an isosmotic condition ( 290 + / - 10 mmol/kg ) served as a control .
	manualset3
107418	2	402784	5	NULL	NULL	0	NULL	hyposmotic conditions	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Medium osmolality was altered to simulate hyposmotic ( 190 + / - 10 mmol/kg ) or hyperosmotic conditions ( 400 + / - 10 mmol/kg ) , whereas an isosmotic condition ( 290 + / - 10 mmol/kg ) served as a control .
	manualset3
107419	3	402784	5	NULL	NULL	0	NULL	190 + / - 10 mmol/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Medium osmolality was altered to simulate hyposmotic ( 190 + / - 10 mmol/kg ) or hyperosmotic conditions ( 400 + / - 10 mmol/kg ) , whereas an isosmotic condition ( 290 + / - 10 mmol/kg ) served as a control .
	manualset3
107420	4	402784	5	NULL	NULL	0	NULL	hyperosmotic conditions	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Medium osmolality was altered to simulate hyposmotic ( 190 + / - 10 mmol/kg ) or hyperosmotic conditions ( 400 + / - 10 mmol/kg ) , whereas an isosmotic condition ( 290 + / - 10 mmol/kg ) served as a control .
	manualset3
107421	5	402784	5	NULL	NULL	0	NULL	400 + / - 10 mmol/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Medium osmolality was altered to simulate hyposmotic ( 190 + / - 10 mmol/kg ) or hyperosmotic conditions ( 400 + / - 10 mmol/kg ) , whereas an isosmotic condition ( 290 + / - 10 mmol/kg ) served as a control .
	manualset3
107422	6	402784	5	NULL	NULL	0	NULL	isosmotic condition	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Medium osmolality was altered to simulate hyposmotic ( 190 + / - 10 mmol/kg ) or hyperosmotic conditions ( 400 + / - 10 mmol/kg ) , whereas an isosmotic condition ( 290 + / - 10 mmol/kg ) served as a control .
	manualset3
107423	7	402784	5	NULL	NULL	0	NULL	290 + / - 10 mmol/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Medium osmolality was altered to simulate hyposmotic ( 190 + / - 10 mmol/kg ) or hyperosmotic conditions ( 400 + / - 10 mmol/kg ) , whereas an isosmotic condition ( 290 + / - 10 mmol/kg ) served as a control .
	manualset3
107424	1	402785	5	NULL	NULL	0	NULL	Medullary CSA	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Medullary CSA was larger with age ( approximately 5 to 65 % ) in both bones but approximately 15 to 440 % greater in the tibia than fibula .
	manualset3
107425	2	402785	5	NULL	NULL	NULL	NULL	age 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Medullary CSA was larger with age ( approximately 5 to 65 % ) in both bones but approximately 15 to 440 % greater in the tibia than fibula .
	manualset3
107426	3	402785	5	NULL	NULL	0	NULL	5 to 65 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Medullary CSA was larger with age ( approximately 5 to 65 % ) in both bones but approximately 15 to 440 % greater in the tibia than fibula .
	manualset3
107427	4	402785	5	NULL	NULL	0	NULL	bones 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Medullary CSA was larger with age ( approximately 5 to 65 % ) in both bones but approximately 15 to 440 % greater in the tibia than fibula .
	manualset3
107428	5	402785	5	NULL	NULL	0	NULL	15 to 440 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Medullary CSA was larger with age ( approximately 5 to 65 % ) in both bones but approximately 15 to 440 % greater in the tibia than fibula .
	manualset3
107429	6	402785	5	NULL	NULL	0	NULL	tibia 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Medullary CSA was larger with age ( approximately 5 to 65 % ) in both bones but approximately 15 to 440 % greater in the tibia than fibula .
	manualset3
107430	7	402785	5	NULL	NULL	0	NULL	fibula 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Medullary CSA was larger with age ( approximately 5 to 65 % ) in both bones but approximately 15 to 440 % greater in the tibia than fibula .
	manualset3
107431	1	402786	5	NULL	NULL	0	NULL	Megafauna 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Megafauna died from big kill , not big chill .
	manualset3
107432	2	402786	5	NULL	NULL	NULL	NULL	chill 	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Megafauna died from big kill , not big chill .
	manualset3
107433	1	402787	5	NULL	NULL	0	NULL	Megakaryocytopoiesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Megakaryocytopoiesis and granulopoiesis after murine cytomegalovirus infection .
	manualset3
107434	2	402787	5	NULL	NULL	0	NULL	granulopoiesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Megakaryocytopoiesis and granulopoiesis after murine cytomegalovirus infection .
	manualset3
107435	3	402787	5	NULL	NULL	0	NULL	murine cytomegalovirus infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Megakaryocytopoiesis and granulopoiesis after murine cytomegalovirus infection .
	manualset3
107436	1	402788	5	NULL	NULL	0	NULL	bone marrow biopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A bone marrow biopsy allowed the diagnosis of an initial stage of `` hairy cells leukemia . ''
	manualset3
107437	2	402788	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A bone marrow biopsy allowed the diagnosis of an initial stage of `` hairy cells leukemia . ''
	manualset3
107438	3	402788	5	NULL	NULL	0	NULL	initial stage 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	A bone marrow biopsy allowed the diagnosis of an initial stage of `` hairy cells leukemia . ''
	manualset3
107439	4	402788	5	NULL	NULL	0	NULL	hairy cells leukemia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A bone marrow biopsy allowed the diagnosis of an initial stage of `` hairy cells leukemia . ''
	manualset3
107440	1	402789	5	NULL	NULL	0	NULL	Meizothrombin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Meizothrombin and the B-chain of thrombin were the only prothrombin fragments detectable .
	manualset3
107441	2	402789	5	NULL	NULL	0	NULL	B-chain 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Meizothrombin and the B-chain of thrombin were the only prothrombin fragments detectable .
	manualset3
107442	3	402789	5	NULL	NULL	0	NULL	thrombin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Meizothrombin and the B-chain of thrombin were the only prothrombin fragments detectable .
	manualset3
107443	4	402789	5	NULL	NULL	0	NULL	prothrombin fragments	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Meizothrombin and the B-chain of thrombin were the only prothrombin fragments detectable .
	manualset3
107444	1	402790	5	NULL	NULL	0	NULL	Mel frequency cepstral coefficients 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mel frequency cepstral coefficients were extracted from them using 15 ms frames and served as training input to the hybrid model setup .
	manualset3
107445	2	402790	5	NULL	NULL	0	NULL	15 ms frames	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mel frequency cepstral coefficients were extracted from them using 15 ms frames and served as training input to the hybrid model setup .
	manualset3
107446	3	402790	5	NULL	NULL	0	NULL	training input	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mel frequency cepstral coefficients were extracted from them using 15 ms frames and served as training input to the hybrid model setup .
	manualset3
107447	4	402790	5	NULL	NULL	0	NULL	hybrid model setup	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Mel frequency cepstral coefficients were extracted from them using 15 ms frames and served as training input to the hybrid model setup .
	manualset3
107448	1	402791	5	NULL	NULL	0	NULL	Melanomas 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Melanomas ( cultured cells or tumor tissue ) were shown to have GD3 and GM3 as major gangliosides .
	manualset3
107449	2	402791	5	NULL	NULL	0	NULL	cultured cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Melanomas ( cultured cells or tumor tissue ) were shown to have GD3 and GM3 as major gangliosides .
	manualset3
107450	3	402791	5	NULL	NULL	NULL	NULL	tumor tissue	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Melanomas ( cultured cells or tumor tissue ) were shown to have GD3 and GM3 as major gangliosides .
	manualset3
107451	4	402791	5	NULL	NULL	0	NULL	GD3 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Melanomas ( cultured cells or tumor tissue ) were shown to have GD3 and GM3 as major gangliosides .
	manualset3
107452	5	402791	5	NULL	NULL	0	NULL	GM3 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Melanomas ( cultured cells or tumor tissue ) were shown to have GD3 and GM3 as major gangliosides .
	manualset3
107453	6	402791	5	NULL	NULL	0	NULL	major gangliosides 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Melanomas ( cultured cells or tumor tissue ) were shown to have GD3 and GM3 as major gangliosides .
	manualset3
107454	1	402792	5	NULL	NULL	0	NULL	Melanosome formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Melanosome formation in the goldfish : the role of multivesicular bodies .
	manualset3
107455	2	402792	5	NULL	NULL	0	NULL	goldfish 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Melanosome formation in the goldfish : the role of multivesicular bodies .
	manualset3
107456	3	402792	5	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Melanosome formation in the goldfish : the role of multivesicular bodies .
	manualset3
107457	4	402792	5	NULL	NULL	0	NULL	multivesicular bodies	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Melanosome formation in the goldfish : the role of multivesicular bodies .
	manualset3
107458	1	402793	5	NULL	NULL	NULL	NULL	Melatonin 	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Melatonin , 2-iodomelatonin , and 2-chloromelatonin injected 3 h before lights off for 16 days ( 17-34 days of age ) significantly inhibited testis growth compared to vehicle-injected hamsters .
	manualset3
107459	2	402793	5	NULL	NULL	0	NULL	2-iodomelatonin	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin , 2-iodomelatonin , and 2-chloromelatonin injected 3 h before lights off for 16 days ( 17-34 days of age ) significantly inhibited testis growth compared to vehicle-injected hamsters .
	manualset3
107460	3	402793	5	NULL	NULL	0	NULL	2-chloromelatonin	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin , 2-iodomelatonin , and 2-chloromelatonin injected 3 h before lights off for 16 days ( 17-34 days of age ) significantly inhibited testis growth compared to vehicle-injected hamsters .
	manualset3
107461	4	402793	5	NULL	NULL	0	NULL	3 h 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin , 2-iodomelatonin , and 2-chloromelatonin injected 3 h before lights off for 16 days ( 17-34 days of age ) significantly inhibited testis growth compared to vehicle-injected hamsters .
	manualset3
107462	5	402793	5	NULL	NULL	0	NULL	16 days	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin , 2-iodomelatonin , and 2-chloromelatonin injected 3 h before lights off for 16 days ( 17-34 days of age ) significantly inhibited testis growth compared to vehicle-injected hamsters .
	manualset3
107463	6	402793	5	NULL	NULL	0	NULL	17-34 days	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin , 2-iodomelatonin , and 2-chloromelatonin injected 3 h before lights off for 16 days ( 17-34 days of age ) significantly inhibited testis growth compared to vehicle-injected hamsters .
	manualset3
107464	7	402793	5	NULL	NULL	0	NULL	age 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin , 2-iodomelatonin , and 2-chloromelatonin injected 3 h before lights off for 16 days ( 17-34 days of age ) significantly inhibited testis growth compared to vehicle-injected hamsters .
	manualset3
107465	8	402793	5	NULL	NULL	0	NULL	testis growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin , 2-iodomelatonin , and 2-chloromelatonin injected 3 h before lights off for 16 days ( 17-34 days of age ) significantly inhibited testis growth compared to vehicle-injected hamsters .
	manualset3
107466	9	402793	5	NULL	NULL	0	NULL	vehicle-injected hamsters	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin , 2-iodomelatonin , and 2-chloromelatonin injected 3 h before lights off for 16 days ( 17-34 days of age ) significantly inhibited testis growth compared to vehicle-injected hamsters .
	manualset3
107467	1	402794	5	NULL	NULL	0	NULL	Melatonin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin , a pineal hormone , is known to be an important neurohormonal factor involved in the timing of reproductive events which occur seasonally in various mammalian species .
	manualset3
107468	2	402794	5	NULL	NULL	0	NULL	pineal hormone	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin , a pineal hormone , is known to be an important neurohormonal factor involved in the timing of reproductive events which occur seasonally in various mammalian species .
	manualset3
107469	3	402794	5	NULL	NULL	0	NULL	neurohormonal factor	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin , a pineal hormone , is known to be an important neurohormonal factor involved in the timing of reproductive events which occur seasonally in various mammalian species .
	manualset3
107470	4	402794	5	NULL	NULL	0	NULL	reproductive events 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin , a pineal hormone , is known to be an important neurohormonal factor involved in the timing of reproductive events which occur seasonally in various mammalian species .
	manualset3
107471	5	402794	5	NULL	NULL	0	NULL	mammalian species 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin , a pineal hormone , is known to be an important neurohormonal factor involved in the timing of reproductive events which occur seasonally in various mammalian species .
	manualset3
107472	1	402795	5	NULL	NULL	0	NULL	Melatonin effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin effect on serotonin uptake and release in rat platelets : diurnal variation in responsiveness .
	manualset3
107473	2	402795	5	NULL	NULL	0	NULL	serotonin uptake 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin effect on serotonin uptake and release in rat platelets : diurnal variation in responsiveness .
	manualset3
107474	3	402795	5	NULL	NULL	0	NULL	release 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin effect on serotonin uptake and release in rat platelets : diurnal variation in responsiveness .
	manualset3
107475	4	402795	5	NULL	NULL	0	NULL	rat platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin effect on serotonin uptake and release in rat platelets : diurnal variation in responsiveness .
	manualset3
107476	5	402795	5	NULL	NULL	0	NULL	diurnal variation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin effect on serotonin uptake and release in rat platelets : diurnal variation in responsiveness .
	manualset3
107477	6	402795	5	NULL	NULL	0	NULL	responsiveness 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin effect on serotonin uptake and release in rat platelets : diurnal variation in responsiveness .
	manualset3
107478	1	402796	5	NULL	NULL	0	NULL	branched pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A branched pathway governing the activation of a developmental transcription factor by regulated intramembrane proteolysis .
	manualset3
107479	2	402796	5	NULL	NULL	0	NULL	activation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A branched pathway governing the activation of a developmental transcription factor by regulated intramembrane proteolysis .
	manualset3
107480	3	402796	5	NULL	NULL	0	NULL	developmental transcription factor	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A branched pathway governing the activation of a developmental transcription factor by regulated intramembrane proteolysis .
	manualset3
107481	4	402796	5	NULL	NULL	0	NULL	regulated intramembrane proteolysis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A branched pathway governing the activation of a developmental transcription factor by regulated intramembrane proteolysis .
	manualset3
107482	1	402797	5	NULL	NULL	0	NULL	Melatonin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin protected both a wild type or demi strain and a demi/dark crossed strain of mink from AD .
	manualset3
107483	2	402797	5	NULL	NULL	0	NULL	wild type mink	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin protected both a wild type or demi strain and a demi/dark crossed strain of mink from AD .
	manualset3
107484	3	402797	5	NULL	NULL	0	NULL	demi strain mink	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin protected both a wild type or demi strain and a demi/dark crossed strain of mink from AD .
	manualset3
107485	4	402797	5	NULL	NULL	0	NULL	demi/dark crossed strain of mink	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin protected both a wild type or demi strain and a demi/dark crossed strain of mink from AD .
	manualset3
107486	5	402797	5	NULL	NULL	0	NULL	AD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Melatonin protected both a wild type or demi strain and a demi/dark crossed strain of mink from AD .
	manualset3
107487	1	402798	5	NULL	NULL	0	NULL	Members of a diverse set of enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of a diverse set of enzymes referred to as N-acyl amino acid synthases are responsible for the production of all metagenome-derived N-acyl amino acids characterized to date .
	manualset3
107488	2	402798	5	NULL	NULL	0	NULL	N-acyl amino acid synthases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of a diverse set of enzymes referred to as N-acyl amino acid synthases are responsible for the production of all metagenome-derived N-acyl amino acids characterized to date .
	manualset3
107489	3	402798	5	NULL	NULL	0	NULL	production 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of a diverse set of enzymes referred to as N-acyl amino acid synthases are responsible for the production of all metagenome-derived N-acyl amino acids characterized to date .
	manualset3
107490	4	402798	5	NULL	NULL	0	NULL	metagenome-derived N-acyl amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of a diverse set of enzymes referred to as N-acyl amino acid synthases are responsible for the production of all metagenome-derived N-acyl amino acids characterized to date .
	manualset3
107491	1	402799	5	NULL	NULL	0	NULL	Members of the Fusarium solani species complex	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of the Fusarium solani species complex are agents of human mycoses , also affecting plants and other animals .
	manualset3
107492	2	402799	5	NULL	NULL	0	NULL	agents 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of the Fusarium solani species complex are agents of human mycoses , also affecting plants and other animals .
	manualset3
107493	3	402799	5	NULL	NULL	0	NULL	human mycoses	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of the Fusarium solani species complex are agents of human mycoses , also affecting plants and other animals .
	manualset3
107494	4	402799	5	NULL	NULL	0	NULL	plants 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of the Fusarium solani species complex are agents of human mycoses , also affecting plants and other animals .
	manualset3
107495	5	402799	5	NULL	NULL	0	NULL	animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of the Fusarium solani species complex are agents of human mycoses , also affecting plants and other animals .
	manualset3
107496	1	402800	5	NULL	NULL	0	NULL	Members of the aquaporin ( AQP ) water channel family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of the aquaporin ( AQP ) water channel family are widely distributed in various tissues and contribute to the water permeability of epithelial and endothelial cells .
	manualset3
107497	2	402800	5	NULL	NULL	0	NULL	various tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of the aquaporin ( AQP ) water channel family are widely distributed in various tissues and contribute to the water permeability of epithelial and endothelial cells .
	manualset3
107498	3	402800	5	NULL	NULL	0	NULL	water permeability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of the aquaporin ( AQP ) water channel family are widely distributed in various tissues and contribute to the water permeability of epithelial and endothelial cells .
	manualset3
107499	4	402800	5	NULL	NULL	0	NULL	epithelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of the aquaporin ( AQP ) water channel family are widely distributed in various tissues and contribute to the water permeability of epithelial and endothelial cells .
	manualset3
107500	5	402800	5	NULL	NULL	0	NULL	endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of the aquaporin ( AQP ) water channel family are widely distributed in various tissues and contribute to the water permeability of epithelial and endothelial cells .
	manualset3
107501	1	402801	5	NULL	NULL	0	NULL	Members of the transient receptor potential ( TRP ) family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of the transient receptor potential ( TRP ) family for which mRNA can be demonstrated in neutrophil granulocytes with RT-PCR include TRPC6 ( as only `` short '' TRP ) , TRPM2 , TRPV1 , TRPV2 , TRPV5 and TRPV6 .
	manualset3
107502	2	402801	5	NULL	NULL	0	NULL	mRNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of the transient receptor potential ( TRP ) family for which mRNA can be demonstrated in neutrophil granulocytes with RT-PCR include TRPC6 ( as only `` short '' TRP ) , TRPM2 , TRPV1 , TRPV2 , TRPV5 and TRPV6 .
	manualset3
107503	3	402801	5	NULL	NULL	0	NULL	neutrophil granulocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of the transient receptor potential ( TRP ) family for which mRNA can be demonstrated in neutrophil granulocytes with RT-PCR include TRPC6 ( as only `` short '' TRP ) , TRPM2 , TRPV1 , TRPV2 , TRPV5 and TRPV6 .
	manualset3
107504	4	402801	5	NULL	NULL	0	NULL	RT-PCR 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of the transient receptor potential ( TRP ) family for which mRNA can be demonstrated in neutrophil granulocytes with RT-PCR include TRPC6 ( as only `` short '' TRP ) , TRPM2 , TRPV1 , TRPV2 , TRPV5 and TRPV6 .
	manualset3
107505	5	402801	5	NULL	NULL	0	NULL	TRPC6 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of the transient receptor potential ( TRP ) family for which mRNA can be demonstrated in neutrophil granulocytes with RT-PCR include TRPC6 ( as only `` short '' TRP ) , TRPM2 , TRPV1 , TRPV2 , TRPV5 and TRPV6 .
	manualset3
107506	6	402801	5	NULL	NULL	0	NULL	`` short '' TRP	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of the transient receptor potential ( TRP ) family for which mRNA can be demonstrated in neutrophil granulocytes with RT-PCR include TRPC6 ( as only `` short '' TRP ) , TRPM2 , TRPV1 , TRPV2 , TRPV5 and TRPV6 .
	manualset3
107507	7	402801	5	NULL	NULL	0	NULL	TRPM2	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of the transient receptor potential ( TRP ) family for which mRNA can be demonstrated in neutrophil granulocytes with RT-PCR include TRPC6 ( as only `` short '' TRP ) , TRPM2 , TRPV1 , TRPV2 , TRPV5 and TRPV6 .
	manualset3
107508	8	402801	5	NULL	NULL	0	NULL	TRPV1 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of the transient receptor potential ( TRP ) family for which mRNA can be demonstrated in neutrophil granulocytes with RT-PCR include TRPC6 ( as only `` short '' TRP ) , TRPM2 , TRPV1 , TRPV2 , TRPV5 and TRPV6 .
	manualset3
107509	9	402801	5	NULL	NULL	0	NULL	TRPV2 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of the transient receptor potential ( TRP ) family for which mRNA can be demonstrated in neutrophil granulocytes with RT-PCR include TRPC6 ( as only `` short '' TRP ) , TRPM2 , TRPV1 , TRPV2 , TRPV5 and TRPV6 .
	manualset3
107510	10	402801	5	NULL	NULL	0	NULL	TRPV5 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of the transient receptor potential ( TRP ) family for which mRNA can be demonstrated in neutrophil granulocytes with RT-PCR include TRPC6 ( as only `` short '' TRP ) , TRPM2 , TRPV1 , TRPV2 , TRPV5 and TRPV6 .
	manualset3
107511	11	402801	5	NULL	NULL	0	NULL	TRPV6 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of the transient receptor potential ( TRP ) family for which mRNA can be demonstrated in neutrophil granulocytes with RT-PCR include TRPC6 ( as only `` short '' TRP ) , TRPM2 , TRPV1 , TRPV2 , TRPV5 and TRPV6 .
	manualset3
107512	1	402802	5	NULL	NULL	0	NULL	Membrane depolarization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Membrane depolarization of cultured myometrial cells from a holding potential of -50 to +70 mV in 10-mV steps under voltage-clamp conditions ( whole cell mode ) activated K + outward currents ( IK ) .
	manualset3
107513	2	402802	5	NULL	NULL	0	NULL	cultured myometrial cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Membrane depolarization of cultured myometrial cells from a holding potential of -50 to +70 mV in 10-mV steps under voltage-clamp conditions ( whole cell mode ) activated K + outward currents ( IK ) .
	manualset3
107514	3	402802	5	NULL	NULL	0	NULL	holding potential	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Membrane depolarization of cultured myometrial cells from a holding potential of -50 to +70 mV in 10-mV steps under voltage-clamp conditions ( whole cell mode ) activated K + outward currents ( IK ) .
	manualset3
107515	4	402802	5	NULL	NULL	0	NULL	-50 to +70 mV	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Membrane depolarization of cultured myometrial cells from a holding potential of -50 to +70 mV in 10-mV steps under voltage-clamp conditions ( whole cell mode ) activated K + outward currents ( IK ) .
	manualset3
107516	5	402802	5	NULL	NULL	0	NULL	10-mV steps	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Membrane depolarization of cultured myometrial cells from a holding potential of -50 to +70 mV in 10-mV steps under voltage-clamp conditions ( whole cell mode ) activated K + outward currents ( IK ) .
	manualset3
107517	6	402802	5	NULL	NULL	0	NULL	voltage-clamp conditions	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Membrane depolarization of cultured myometrial cells from a holding potential of -50 to +70 mV in 10-mV steps under voltage-clamp conditions ( whole cell mode ) activated K + outward currents ( IK ) .
	manualset3
107518	7	402802	5	NULL	NULL	0	NULL	whole cell mode	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Membrane depolarization of cultured myometrial cells from a holding potential of -50 to +70 mV in 10-mV steps under voltage-clamp conditions ( whole cell mode ) activated K + outward currents ( IK ) .
	manualset3
107519	8	402802	5	NULL	NULL	0	NULL	activated K + outward currents ( IK )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Membrane depolarization of cultured myometrial cells from a holding potential of -50 to +70 mV in 10-mV steps under voltage-clamp conditions ( whole cell mode ) activated K + outward currents ( IK ) .
	manualset3
107520	1	402803	5	NULL	NULL	0	NULL	Membrane sequestration 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Membrane sequestration of the signal transduction protein GlnK by the ammonium transporter AmtB .
	manualset3
107521	2	402803	5	NULL	NULL	0	NULL	signal transduction protein GlnK 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Membrane sequestration of the signal transduction protein GlnK by the ammonium transporter AmtB .
	manualset3
107522	3	402803	5	NULL	NULL	0	NULL	ammonium transporter AmtB	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Membrane sequestration of the signal transduction protein GlnK by the ammonium transporter AmtB .
	manualset3
107523	1	402804	5	NULL	NULL	0	NULL	brief discussion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A brief discussion on the application of these results towards the inversion of sediment attenuation is given .
	manualset3
107524	2	402804	5	NULL	NULL	0	NULL	application 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A brief discussion on the application of these results towards the inversion of sediment attenuation is given .
	manualset3
107525	3	402804	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A brief discussion on the application of these results towards the inversion of sediment attenuation is given .
	manualset3
107526	4	402804	5	NULL	NULL	0	NULL	inversion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A brief discussion on the application of these results towards the inversion of sediment attenuation is given .
	manualset3
107527	5	402804	5	NULL	NULL	0	NULL	sediment attenuation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A brief discussion on the application of these results towards the inversion of sediment attenuation is given .
	manualset3
107528	1	402805	5	NULL	NULL	0	NULL	Memory 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Memory for the two types of activities varied with cue condition and with the presence of the end product .
	manualset3
107529	2	402805	5	NULL	NULL	0	NULL	two types of activities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Memory for the two types of activities varied with cue condition and with the presence of the end product .
	manualset3
107530	3	402805	5	NULL	NULL	0	NULL	cue condition	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Memory for the two types of activities varied with cue condition and with the presence of the end product .
	manualset3
107531	4	402805	5	NULL	NULL	0	NULL	end product 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Memory for the two types of activities varied with cue condition and with the presence of the end product .
	manualset3
107532	5	402805	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Memory for the two types of activities varied with cue condition and with the presence of the end product .
	manualset3
107533	1	402806	5	NULL	NULL	0	NULL	Memory loss 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Memory loss did not seem to be directly responsible of the symptom , while personality features and social cultural models seemed to have a definite valence in the development of confabulation of denial .
	manualset3
107534	2	402806	5	NULL	NULL	0	NULL	symptom 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Memory loss did not seem to be directly responsible of the symptom , while personality features and social cultural models seemed to have a definite valence in the development of confabulation of denial .
	manualset3
107535	3	402806	5	NULL	NULL	0	NULL	personality features 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Memory loss did not seem to be directly responsible of the symptom , while personality features and social cultural models seemed to have a definite valence in the development of confabulation of denial .
	manualset3
107536	4	402806	5	NULL	NULL	NULL	NULL	social cultural models	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Memory loss did not seem to be directly responsible of the symptom , while personality features and social cultural models seemed to have a definite valence in the development of confabulation of denial .
	manualset3
107537	5	402806	5	NULL	NULL	0	NULL	definite valence 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Memory loss did not seem to be directly responsible of the symptom , while personality features and social cultural models seemed to have a definite valence in the development of confabulation of denial .
	manualset3
107538	6	402806	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Memory loss did not seem to be directly responsible of the symptom , while personality features and social cultural models seemed to have a definite valence in the development of confabulation of denial .
	manualset3
107539	7	402806	5	NULL	NULL	0	NULL	confabulation of denial	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Memory loss did not seem to be directly responsible of the symptom , while personality features and social cultural models seemed to have a definite valence in the development of confabulation of denial .
	manualset3
107540	1	402807	5	NULL	NULL	0	NULL	Men 's knowledge	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Men 's knowledge and beliefs about colorectal cancer and 3 screenings : education , race , and screening status .
	manualset3
107541	2	402807	5	NULL	NULL	0	NULL	beliefs 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Men 's knowledge and beliefs about colorectal cancer and 3 screenings : education , race , and screening status .
	manualset3
107542	3	402807	5	NULL	NULL	0	NULL	colorectal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Men 's knowledge and beliefs about colorectal cancer and 3 screenings : education , race , and screening status .
	manualset3
107543	4	402807	5	NULL	NULL	0	NULL	3 screenings	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Men 's knowledge and beliefs about colorectal cancer and 3 screenings : education , race , and screening status .
	manualset3
107544	5	402807	5	NULL	NULL	0	NULL	education 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Men 's knowledge and beliefs about colorectal cancer and 3 screenings : education , race , and screening status .
	manualset3
107545	6	402807	5	NULL	NULL	NULL	NULL	race	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Men 's knowledge and beliefs about colorectal cancer and 3 screenings : education , race , and screening status .
	manualset3
107546	7	402807	5	NULL	NULL	0	NULL	screening status	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Men 's knowledge and beliefs about colorectal cancer and 3 screenings : education , race , and screening status .
	manualset3
107547	1	402808	5	NULL	NULL	0	NULL	Men 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Men who have sex with transgender women are a potentially high-risk population for HIV and other sexually transmitted infections ( STIs ) .
	manualset3
107548	2	402808	5	NULL	NULL	0	NULL	sex 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Men who have sex with transgender women are a potentially high-risk population for HIV and other sexually transmitted infections ( STIs ) .
	manualset3
107549	3	402808	5	NULL	NULL	0	NULL	transgender women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Men who have sex with transgender women are a potentially high-risk population for HIV and other sexually transmitted infections ( STIs ) .
	manualset3
107550	4	402808	5	NULL	NULL	0	NULL	potentially high-risk population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Men who have sex with transgender women are a potentially high-risk population for HIV and other sexually transmitted infections ( STIs ) .
	manualset3
107551	5	402808	5	NULL	NULL	0	NULL	HIV infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Men who have sex with transgender women are a potentially high-risk population for HIV and other sexually transmitted infections ( STIs ) .
	manualset3
107552	6	402808	5	NULL	NULL	0	NULL	sexually transmitted infections ( STIs )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Men who have sex with transgender women are a potentially high-risk population for HIV and other sexually transmitted infections ( STIs ) .
	manualset3
107553	1	402809	5	NULL	NULL	0	NULL	brief review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A brief review of laparoscopic appendectomy : the issues and the evidence .
	manualset3
107554	2	402809	5	NULL	NULL	0	NULL	laparoscopic appendectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A brief review of laparoscopic appendectomy : the issues and the evidence .
	manualset3
107555	3	402809	5	NULL	NULL	NULL	NULL	issues 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A brief review of laparoscopic appendectomy : the issues and the evidence .
	manualset3
107556	4	402809	5	NULL	NULL	0	NULL	evidence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A brief review of laparoscopic appendectomy : the issues and the evidence .
	manualset3
107557	1	402810	5	NULL	NULL	NULL	NULL	Menadione toxicity	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Menadione toxicity in Saccharomyces cerevisiae cells : activation by conjugation with glutathione .
	manualset3
107558	2	402810	5	NULL	NULL	0	NULL	Saccharomyces cerevisiae cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Menadione toxicity in Saccharomyces cerevisiae cells : activation by conjugation with glutathione .
	manualset3
107559	3	402810	5	NULL	NULL	0	NULL	activation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Menadione toxicity in Saccharomyces cerevisiae cells : activation by conjugation with glutathione .
	manualset3
107560	4	402810	5	NULL	NULL	0	NULL	conjugation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Menadione toxicity in Saccharomyces cerevisiae cells : activation by conjugation with glutathione .
	manualset3
107561	5	402810	5	NULL	NULL	0	NULL	glutathione 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Menadione toxicity in Saccharomyces cerevisiae cells : activation by conjugation with glutathione .
	manualset3
107562	1	402811	5	NULL	NULL	0	NULL	Meningitis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Meningitis due to Listeria monocytogenes .
	manualset3
107563	2	402811	5	NULL	NULL	0	NULL	Listeria monocytogenes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Meningitis due to Listeria monocytogenes .
	manualset3
107564	1	402812	5	NULL	NULL	0	NULL	Mental impairments	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mental or physical impairments , such as dementing illnesses , or impaired dexterity as a result of arthritis or stroke , can impair an adult 's ability to perform adequate oral self-care .
	manualset3
107565	2	402812	5	NULL	NULL	0	NULL	physical impairments	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mental or physical impairments , such as dementing illnesses , or impaired dexterity as a result of arthritis or stroke , can impair an adult 's ability to perform adequate oral self-care .
	manualset3
107566	3	402812	5	NULL	NULL	0	NULL	dementing illnesses	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mental or physical impairments , such as dementing illnesses , or impaired dexterity as a result of arthritis or stroke , can impair an adult 's ability to perform adequate oral self-care .
	manualset3
107567	4	402812	5	NULL	NULL	0	NULL	impaired dexterity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mental or physical impairments , such as dementing illnesses , or impaired dexterity as a result of arthritis or stroke , can impair an adult 's ability to perform adequate oral self-care .
	manualset3
107568	5	402812	5	NULL	NULL	0	NULL	result 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mental or physical impairments , such as dementing illnesses , or impaired dexterity as a result of arthritis or stroke , can impair an adult 's ability to perform adequate oral self-care .
	manualset3
107569	6	402812	5	NULL	NULL	0	NULL	arthritis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mental or physical impairments , such as dementing illnesses , or impaired dexterity as a result of arthritis or stroke , can impair an adult 's ability to perform adequate oral self-care .
	manualset3
107570	7	402812	5	NULL	NULL	0	NULL	stroke 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mental or physical impairments , such as dementing illnesses , or impaired dexterity as a result of arthritis or stroke , can impair an adult 's ability to perform adequate oral self-care .
	manualset3
107571	8	402812	5	NULL	NULL	0	NULL	adult 's ability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mental or physical impairments , such as dementing illnesses , or impaired dexterity as a result of arthritis or stroke , can impair an adult 's ability to perform adequate oral self-care .
	manualset3
107572	9	402812	5	NULL	NULL	0	NULL	adequate oral self-care	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mental or physical impairments , such as dementing illnesses , or impaired dexterity as a result of arthritis or stroke , can impair an adult 's ability to perform adequate oral self-care .
	manualset3
107573	1	402813	5	NULL	NULL	0	NULL	Mental retardation locus	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Mental retardation locus in Xp21 chromosome microdeletion .
	manualset3
107574	2	402813	5	NULL	NULL	0	NULL	Xp21 chromosome microdeletion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mental retardation locus in Xp21 chromosome microdeletion .
	manualset3
107575	1	402814	5	NULL	NULL	0	NULL	Mental retardation/intellectual disability	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mental retardation/intellectual disability is a devastating neurodevelopmental disorder with serious impact on affected individuals and their families , as well as on health and social services .
	manualset3
107576	2	402814	5	NULL	NULL	0	NULL	neurodevelopmental disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mental retardation/intellectual disability is a devastating neurodevelopmental disorder with serious impact on affected individuals and their families , as well as on health and social services .
	manualset3
107577	3	402814	5	NULL	NULL	0	NULL	serious impact 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mental retardation/intellectual disability is a devastating neurodevelopmental disorder with serious impact on affected individuals and their families , as well as on health and social services .
	manualset3
107578	4	402814	5	NULL	NULL	0	NULL	affected individuals 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mental retardation/intellectual disability is a devastating neurodevelopmental disorder with serious impact on affected individuals and their families , as well as on health and social services .
	manualset3
107579	5	402814	5	NULL	NULL	0	NULL	families 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mental retardation/intellectual disability is a devastating neurodevelopmental disorder with serious impact on affected individuals and their families , as well as on health and social services .
	manualset3
107580	6	402814	5	NULL	NULL	0	NULL	health 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mental retardation/intellectual disability is a devastating neurodevelopmental disorder with serious impact on affected individuals and their families , as well as on health and social services .
	manualset3
107581	7	402814	5	NULL	NULL	0	NULL	social services	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mental retardation/intellectual disability is a devastating neurodevelopmental disorder with serious impact on affected individuals and their families , as well as on health and social services .
	manualset3
107582	1	402815	5	NULL	NULL	0	NULL	Meprin metalloproteinases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Meprin metalloproteinases have been implicated in the susceptibility to and progression of diabetic nephropathy and inflammatory bowel diseases .
	manualset3
107583	2	402815	5	NULL	NULL	0	NULL	susceptibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Meprin metalloproteinases have been implicated in the susceptibility to and progression of diabetic nephropathy and inflammatory bowel diseases .
	manualset3
107584	3	402815	5	NULL	NULL	0	NULL	progression 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Meprin metalloproteinases have been implicated in the susceptibility to and progression of diabetic nephropathy and inflammatory bowel diseases .
	manualset3
107585	4	402815	5	NULL	NULL	0	NULL	diabetic nephropathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Meprin metalloproteinases have been implicated in the susceptibility to and progression of diabetic nephropathy and inflammatory bowel diseases .
	manualset3
107586	5	402815	5	NULL	NULL	0	NULL	inflammatory bowel diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Meprin metalloproteinases have been implicated in the susceptibility to and progression of diabetic nephropathy and inflammatory bowel diseases .
	manualset3
107587	1	402816	5	NULL	NULL	0	NULL	Mepyramine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Mepyramine prevented the increase in heart rate but did not affect the chronotropic actions of isoproterenol and glyceryl trinitrate .
	manualset3
107588	2	402816	5	NULL	NULL	0	NULL	increase in heart rate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mepyramine prevented the increase in heart rate but did not affect the chronotropic actions of isoproterenol and glyceryl trinitrate .
	manualset3
107589	3	402816	5	NULL	NULL	0	NULL	chronotropic actions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mepyramine prevented the increase in heart rate but did not affect the chronotropic actions of isoproterenol and glyceryl trinitrate .
	manualset3
107590	4	402816	5	NULL	NULL	0	NULL	isoproterenol 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Mepyramine prevented the increase in heart rate but did not affect the chronotropic actions of isoproterenol and glyceryl trinitrate .
	manualset3
107591	5	402816	5	NULL	NULL	0	NULL	glyceryl trinitrate	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Mepyramine prevented the increase in heart rate but did not affect the chronotropic actions of isoproterenol and glyceryl trinitrate .
	manualset3
107592	1	402817	5	NULL	NULL	0	NULL	Mercuric chloride	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Mercuric chloride probably causes oxidant stress by the generation of free-radicals , activating NK-kappaB , a transcription factor for the IL-4 gene .
	manualset3
107593	2	402817	5	NULL	NULL	0	NULL	oxidant stress	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mercuric chloride probably causes oxidant stress by the generation of free-radicals , activating NK-kappaB , a transcription factor for the IL-4 gene .
	manualset3
107594	3	402817	5	NULL	NULL	0	NULL	generation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mercuric chloride probably causes oxidant stress by the generation of free-radicals , activating NK-kappaB , a transcription factor for the IL-4 gene .
	manualset3
107595	4	402817	5	NULL	NULL	0	NULL	free-radicals	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Mercuric chloride probably causes oxidant stress by the generation of free-radicals , activating NK-kappaB , a transcription factor for the IL-4 gene .
	manualset3
107596	5	402817	5	NULL	NULL	NULL	NULL	NK-kappaB , a transcription factor	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mercuric chloride probably causes oxidant stress by the generation of free-radicals , activating NK-kappaB , a transcription factor for the IL-4 gene .
	manualset3
107597	6	402817	5	NULL	NULL	0	NULL	IL-4 gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Mercuric chloride probably causes oxidant stress by the generation of free-radicals , activating NK-kappaB , a transcription factor for the IL-4 gene .
	manualset3
107598	1	402818	5	NULL	NULL	0	NULL	Mercury concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mercury concentration was significantly related to age but not to gender for otter .
	manualset3
107599	2	402818	5	NULL	NULL	0	NULL	age 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mercury concentration was significantly related to age but not to gender for otter .
	manualset3
107600	3	402818	5	NULL	NULL	0	NULL	gender 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mercury concentration was significantly related to age but not to gender for otter .
	manualset3
107601	4	402818	5	NULL	NULL	0	NULL	otter 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mercury concentration was significantly related to age but not to gender for otter .
	manualset3
107602	1	402819	5	NULL	NULL	0	NULL	brief review 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A brief review of the genetics of epilepsy is presented , with emphasis on quality of life issues from the perspective of the daily lives of patients with familial epilepsies and on issues regarding clinical research in such families .
	manualset3
107603	2	402819	5	NULL	NULL	0	NULL	genetics 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A brief review of the genetics of epilepsy is presented , with emphasis on quality of life issues from the perspective of the daily lives of patients with familial epilepsies and on issues regarding clinical research in such families .
	manualset3
107604	3	402819	5	NULL	NULL	0	NULL	epilepsy 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A brief review of the genetics of epilepsy is presented , with emphasis on quality of life issues from the perspective of the daily lives of patients with familial epilepsies and on issues regarding clinical research in such families .
	manualset3
107605	4	402819	5	NULL	NULL	0	NULL	quality of life issues	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A brief review of the genetics of epilepsy is presented , with emphasis on quality of life issues from the perspective of the daily lives of patients with familial epilepsies and on issues regarding clinical research in such families .
	manualset3
107606	5	402819	5	NULL	NULL	0	NULL	perspective 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A brief review of the genetics of epilepsy is presented , with emphasis on quality of life issues from the perspective of the daily lives of patients with familial epilepsies and on issues regarding clinical research in such families .
	manualset3
107607	6	402819	5	NULL	NULL	0	NULL	daily lives 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A brief review of the genetics of epilepsy is presented , with emphasis on quality of life issues from the perspective of the daily lives of patients with familial epilepsies and on issues regarding clinical research in such families .
	manualset3
107608	7	402819	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A brief review of the genetics of epilepsy is presented , with emphasis on quality of life issues from the perspective of the daily lives of patients with familial epilepsies and on issues regarding clinical research in such families .
	manualset3
107609	8	402819	5	NULL	NULL	0	NULL	familial epilepsies	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A brief review of the genetics of epilepsy is presented , with emphasis on quality of life issues from the perspective of the daily lives of patients with familial epilepsies and on issues regarding clinical research in such families .
	manualset3
107610	9	402819	5	NULL	NULL	0	NULL	issues 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A brief review of the genetics of epilepsy is presented , with emphasis on quality of life issues from the perspective of the daily lives of patients with familial epilepsies and on issues regarding clinical research in such families .
	manualset3
107611	10	402819	5	NULL	NULL	0	NULL	clinical research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A brief review of the genetics of epilepsy is presented , with emphasis on quality of life issues from the perspective of the daily lives of patients with familial epilepsies and on issues regarding clinical research in such families .
	manualset3
107612	11	402819	5	NULL	NULL	0	NULL	families 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A brief review of the genetics of epilepsy is presented , with emphasis on quality of life issues from the perspective of the daily lives of patients with familial epilepsies and on issues regarding clinical research in such families .
	manualset3
107613	1	402820	5	NULL	NULL	0	NULL	Mercury wet deposition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mercury wet deposition in rural Korea : concentrations and fluxes .
	manualset3
107614	2	402820	5	NULL	NULL	0	NULL	rural Korea	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Mercury wet deposition in rural Korea : concentrations and fluxes .
	manualset3
107615	3	402820	5	NULL	NULL	0	NULL	concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mercury wet deposition in rural Korea : concentrations and fluxes .
	manualset3
107616	4	402820	5	NULL	NULL	0	NULL	fluxes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mercury wet deposition in rural Korea : concentrations and fluxes .
	manualset3
107617	1	402821	5	NULL	NULL	0	NULL	Mesenchymal stem cells ( MSCs ) 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesenchymal stem cells ( MSCs ) are an alluring therapeutic resource because of their plasticity , immunoregulatory capacity and ease of availability .
	manualset3
107618	2	402821	5	NULL	NULL	NULL	NULL	alluring therapeutic resource	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mesenchymal stem cells ( MSCs ) are an alluring therapeutic resource because of their plasticity , immunoregulatory capacity and ease of availability .
	manualset3
107619	3	402821	5	NULL	NULL	0	NULL	plasticity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesenchymal stem cells ( MSCs ) are an alluring therapeutic resource because of their plasticity , immunoregulatory capacity and ease of availability .
	manualset3
107620	4	402821	5	NULL	NULL	0	NULL	immunoregulatory capacity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesenchymal stem cells ( MSCs ) are an alluring therapeutic resource because of their plasticity , immunoregulatory capacity and ease of availability .
	manualset3
107621	5	402821	5	NULL	NULL	0	NULL	ease of availability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesenchymal stem cells ( MSCs ) are an alluring therapeutic resource because of their plasticity , immunoregulatory capacity and ease of availability .
	manualset3
107622	1	402822	5	NULL	NULL	0	NULL	Mesenchymal stem cells ( MSCs )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesenchymal stem cells ( MSCs ) are multipotent progenitor cells and interest in MSC therapy has been raised by the observation that MSCs are able to modulate immune responses in vitro and in vivo .
	manualset3
107623	2	402822	5	NULL	NULL	0	NULL	multipotent progenitor cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesenchymal stem cells ( MSCs ) are multipotent progenitor cells and interest in MSC therapy has been raised by the observation that MSCs are able to modulate immune responses in vitro and in vivo .
	manualset3
107624	3	402822	5	NULL	NULL	0	NULL	MSC therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesenchymal stem cells ( MSCs ) are multipotent progenitor cells and interest in MSC therapy has been raised by the observation that MSCs are able to modulate immune responses in vitro and in vivo .
	manualset3
107625	4	402822	5	NULL	NULL	0	NULL	observation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesenchymal stem cells ( MSCs ) are multipotent progenitor cells and interest in MSC therapy has been raised by the observation that MSCs are able to modulate immune responses in vitro and in vivo .
	manualset3
107626	5	402822	5	NULL	NULL	0	NULL	MSCs 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesenchymal stem cells ( MSCs ) are multipotent progenitor cells and interest in MSC therapy has been raised by the observation that MSCs are able to modulate immune responses in vitro and in vivo .
	manualset3
107628	7	402822	5	NULL	NULL	0	NULL	immune responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesenchymal stem cells ( MSCs ) are multipotent progenitor cells and interest in MSC therapy has been raised by the observation that MSCs are able to modulate immune responses in vitro and in vivo .
	manualset3
107629	1	402823	5	NULL	NULL	0	NULL	Mesenteric thrombosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesenteric thrombosis associated with thromboangiitis obliterans ; report of case .
	manualset3
107630	2	402823	5	NULL	NULL	0	NULL	thromboangiitis obliterans	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesenteric thrombosis associated with thromboangiitis obliterans ; report of case .
	manualset3
107631	3	402823	5	NULL	NULL	0	NULL	case 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesenteric thrombosis associated with thromboangiitis obliterans ; report of case .
	manualset3
107632	1	402824	5	NULL	NULL	0	NULL	Mesoporous carbons	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesoporous carbons with extremely large pore volume ( approximately 6 cm3/g ) and narrow bimodal pore size distribution were synthesized by using 24 nm silica colloids as template .
	manualset3
107633	2	402824	5	NULL	NULL	0	NULL	extremely large pore volume 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesoporous carbons with extremely large pore volume ( approximately 6 cm3/g ) and narrow bimodal pore size distribution were synthesized by using 24 nm silica colloids as template .
	manualset3
107634	3	402824	5	NULL	NULL	0	NULL	6 cm3/g	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesoporous carbons with extremely large pore volume ( approximately 6 cm3/g ) and narrow bimodal pore size distribution were synthesized by using 24 nm silica colloids as template .
	manualset3
107635	4	402824	5	NULL	NULL	0	NULL	narrow bimodal pore size distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesoporous carbons with extremely large pore volume ( approximately 6 cm3/g ) and narrow bimodal pore size distribution were synthesized by using 24 nm silica colloids as template .
	manualset3
107636	5	402824	5	NULL	NULL	0	NULL	 24 nm silica colloids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesoporous carbons with extremely large pore volume ( approximately 6 cm3/g ) and narrow bimodal pore size distribution were synthesized by using 24 nm silica colloids as template .
	manualset3
107637	6	402824	5	NULL	NULL	0	NULL	template 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesoporous carbons with extremely large pore volume ( approximately 6 cm3/g ) and narrow bimodal pore size distribution were synthesized by using 24 nm silica colloids as template .
	manualset3
107638	1	402825	5	NULL	NULL	0	NULL	Mesothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesothelial cells might be useful for biological revascularization in patients with ischemic heart disease .
	manualset3
107639	2	402825	5	NULL	NULL	0	NULL	biological revascularization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesothelial cells might be useful for biological revascularization in patients with ischemic heart disease .
	manualset3
107640	3	402825	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesothelial cells might be useful for biological revascularization in patients with ischemic heart disease .
	manualset3
107641	4	402825	5	NULL	NULL	0	NULL	ischemic heart disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesothelial cells might be useful for biological revascularization in patients with ischemic heart disease .
	manualset3
107642	1	402826	5	NULL	NULL	0	NULL	Messenger RNA expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Messenger RNA expression of B7-1 and NPHS1 in urinary sediment could be useful to differentiate between minimal-change disease and focal segmental glomerulosclerosis in adult patients .
	manualset3
107643	2	402826	5	NULL	NULL	0	NULL	B7-1	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Messenger RNA expression of B7-1 and NPHS1 in urinary sediment could be useful to differentiate between minimal-change disease and focal segmental glomerulosclerosis in adult patients .
	manualset3
107644	3	402826	5	NULL	NULL	0	NULL	NPHS1 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Messenger RNA expression of B7-1 and NPHS1 in urinary sediment could be useful to differentiate between minimal-change disease and focal segmental glomerulosclerosis in adult patients .
	manualset3
107645	4	402826	5	NULL	NULL	0	NULL	urinary sediment	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Messenger RNA expression of B7-1 and NPHS1 in urinary sediment could be useful to differentiate between minimal-change disease and focal segmental glomerulosclerosis in adult patients .
	manualset3
107646	5	402826	5	NULL	NULL	0	NULL	differentiate 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Messenger RNA expression of B7-1 and NPHS1 in urinary sediment could be useful to differentiate between minimal-change disease and focal segmental glomerulosclerosis in adult patients .
	manualset3
107647	6	402826	5	NULL	NULL	0	NULL	minimal-change disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Messenger RNA expression of B7-1 and NPHS1 in urinary sediment could be useful to differentiate between minimal-change disease and focal segmental glomerulosclerosis in adult patients .
	manualset3
107648	7	402826	5	NULL	NULL	0	NULL	focal segmental glomerulosclerosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Messenger RNA expression of B7-1 and NPHS1 in urinary sediment could be useful to differentiate between minimal-change disease and focal segmental glomerulosclerosis in adult patients .
	manualset3
107649	8	402826	5	NULL	NULL	0	NULL	adult patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Messenger RNA expression of B7-1 and NPHS1 in urinary sediment could be useful to differentiate between minimal-change disease and focal segmental glomerulosclerosis in adult patients .
	manualset3
107650	1	402827	5	NULL	NULL	0	NULL	Metabolic acidosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic acidosis may be related to PEM and MICS due to an increased protein catabolism , decreased protein synthesis , endocrine abnormalities including insulin resistance , decreased serum leptin level , and inflammation among individuals with renal failure .
	manualset3
107651	2	402827	5	NULL	NULL	0	NULL	PEM 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic acidosis may be related to PEM and MICS due to an increased protein catabolism , decreased protein synthesis , endocrine abnormalities including insulin resistance , decreased serum leptin level , and inflammation among individuals with renal failure .
	manualset3
107652	3	402827	5	NULL	NULL	0	NULL	MICS 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic acidosis may be related to PEM and MICS due to an increased protein catabolism , decreased protein synthesis , endocrine abnormalities including insulin resistance , decreased serum leptin level , and inflammation among individuals with renal failure .
	manualset3
107653	4	402827	5	NULL	NULL	0	NULL	increased protein catabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic acidosis may be related to PEM and MICS due to an increased protein catabolism , decreased protein synthesis , endocrine abnormalities including insulin resistance , decreased serum leptin level , and inflammation among individuals with renal failure .
	manualset3
107654	5	402827	5	NULL	NULL	0	NULL	decreased protein synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic acidosis may be related to PEM and MICS due to an increased protein catabolism , decreased protein synthesis , endocrine abnormalities including insulin resistance , decreased serum leptin level , and inflammation among individuals with renal failure .
	manualset3
107655	6	402827	5	NULL	NULL	0	NULL	endocrine abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic acidosis may be related to PEM and MICS due to an increased protein catabolism , decreased protein synthesis , endocrine abnormalities including insulin resistance , decreased serum leptin level , and inflammation among individuals with renal failure .
	manualset3
107656	7	402827	5	NULL	NULL	0	NULL	insulin resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic acidosis may be related to PEM and MICS due to an increased protein catabolism , decreased protein synthesis , endocrine abnormalities including insulin resistance , decreased serum leptin level , and inflammation among individuals with renal failure .
	manualset3
107657	8	402827	5	NULL	NULL	0	NULL	decreased serum leptin level	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic acidosis may be related to PEM and MICS due to an increased protein catabolism , decreased protein synthesis , endocrine abnormalities including insulin resistance , decreased serum leptin level , and inflammation among individuals with renal failure .
	manualset3
107658	9	402827	5	NULL	NULL	0	NULL	inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic acidosis may be related to PEM and MICS due to an increased protein catabolism , decreased protein synthesis , endocrine abnormalities including insulin resistance , decreased serum leptin level , and inflammation among individuals with renal failure .
	manualset3
107659	10	402827	5	NULL	NULL	0	NULL	individuals 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic acidosis may be related to PEM and MICS due to an increased protein catabolism , decreased protein synthesis , endocrine abnormalities including insulin resistance , decreased serum leptin level , and inflammation among individuals with renal failure .
	manualset3
107660	11	402827	5	NULL	NULL	0	NULL	renal failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic acidosis may be related to PEM and MICS due to an increased protein catabolism , decreased protein synthesis , endocrine abnormalities including insulin resistance , decreased serum leptin level , and inflammation among individuals with renal failure .
	manualset3
107661	1	402828	5	NULL	NULL	0	NULL	Metabolic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic activity in the isolated perfused placental lobule was assessed in terms of these tissue metabolites and by measuring protein synthetic rate by means of determining the incorporation of a labeled amino acid .
	manualset3
107662	2	402828	5	NULL	NULL	0	NULL	isolated perfused placental lobule 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic activity in the isolated perfused placental lobule was assessed in terms of these tissue metabolites and by measuring protein synthetic rate by means of determining the incorporation of a labeled amino acid .
	manualset3
107663	3	402828	5	NULL	NULL	0	NULL	tissue metabolites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic activity in the isolated perfused placental lobule was assessed in terms of these tissue metabolites and by measuring protein synthetic rate by means of determining the incorporation of a labeled amino acid .
	manualset3
107664	4	402828	5	NULL	NULL	0	NULL	protein synthetic rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic activity in the isolated perfused placental lobule was assessed in terms of these tissue metabolites and by measuring protein synthetic rate by means of determining the incorporation of a labeled amino acid .
	manualset3
107665	5	402828	5	NULL	NULL	0	NULL	incorporation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic activity in the isolated perfused placental lobule was assessed in terms of these tissue metabolites and by measuring protein synthetic rate by means of determining the incorporation of a labeled amino acid .
	manualset3
107666	6	402828	5	NULL	NULL	0	NULL	labeled amino acid	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic activity in the isolated perfused placental lobule was assessed in terms of these tissue metabolites and by measuring protein synthetic rate by means of determining the incorporation of a labeled amino acid .
	manualset3
107667	1	402829	5	NULL	NULL	0	NULL	Metabolic effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic effects of the major component of bovine growth hormone .
	manualset3
107668	2	402829	5	NULL	NULL	0	NULL	major component of bovine growth hormone	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic effects of the major component of bovine growth hormone .
	manualset3
107669	1	402830	5	NULL	NULL	0	NULL	Metabolic labeling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic labeling with ( 35S ) SO4 ( 2 - ) or ( 35S ) methionine and immunoprecipitation demonstrated that ( 35S ) SO4 ( 2 - ) was efficiently incorporated into PAM proteins that have the noncatalytic exon A region following the monooxygenase domain ( PAM-1 and PAM-4 ) and into a soluble bifunctional PAM protein ( PAM-3 ) .
	manualset3
107670	2	402830	5	NULL	NULL	NULL	NULL	( 35S ) SO4 ( 2 - ) methionine	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Metabolic labeling with ( 35S ) SO4 ( 2 - ) or ( 35S ) methionine and immunoprecipitation demonstrated that ( 35S ) SO4 ( 2 - ) was efficiently incorporated into PAM proteins that have the noncatalytic exon A region following the monooxygenase domain ( PAM-1 and PAM-4 ) and into a soluble bifunctional PAM protein ( PAM-3 ) .
	manualset3
107671	3	402830	5	NULL	NULL	0	NULL	( 35S ) methionine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic labeling with ( 35S ) SO4 ( 2 - ) or ( 35S ) methionine and immunoprecipitation demonstrated that ( 35S ) SO4 ( 2 - ) was efficiently incorporated into PAM proteins that have the noncatalytic exon A region following the monooxygenase domain ( PAM-1 and PAM-4 ) and into a soluble bifunctional PAM protein ( PAM-3 ) .
	manualset3
107672	4	402830	5	NULL	NULL	0	NULL	immunoprecipitation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic labeling with ( 35S ) SO4 ( 2 - ) or ( 35S ) methionine and immunoprecipitation demonstrated that ( 35S ) SO4 ( 2 - ) was efficiently incorporated into PAM proteins that have the noncatalytic exon A region following the monooxygenase domain ( PAM-1 and PAM-4 ) and into a soluble bifunctional PAM protein ( PAM-3 ) .
	manualset3
107673	5	402830	5	NULL	NULL	0	NULL	( 35S ) SO4 ( 2 - ) 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic labeling with ( 35S ) SO4 ( 2 - ) or ( 35S ) methionine and immunoprecipitation demonstrated that ( 35S ) SO4 ( 2 - ) was efficiently incorporated into PAM proteins that have the noncatalytic exon A region following the monooxygenase domain ( PAM-1 and PAM-4 ) and into a soluble bifunctional PAM protein ( PAM-3 ) .
	manualset3
107674	6	402830	5	NULL	NULL	0	NULL	PAM proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic labeling with ( 35S ) SO4 ( 2 - ) or ( 35S ) methionine and immunoprecipitation demonstrated that ( 35S ) SO4 ( 2 - ) was efficiently incorporated into PAM proteins that have the noncatalytic exon A region following the monooxygenase domain ( PAM-1 and PAM-4 ) and into a soluble bifunctional PAM protein ( PAM-3 ) .
	manualset3
107675	7	402830	5	NULL	NULL	0	NULL	noncatalytic exon A region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic labeling with ( 35S ) SO4 ( 2 - ) or ( 35S ) methionine and immunoprecipitation demonstrated that ( 35S ) SO4 ( 2 - ) was efficiently incorporated into PAM proteins that have the noncatalytic exon A region following the monooxygenase domain ( PAM-1 and PAM-4 ) and into a soluble bifunctional PAM protein ( PAM-3 ) .
	manualset3
107676	8	402830	5	NULL	NULL	NULL	NULL	monooxygenase domain 	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Metabolic labeling with ( 35S ) SO4 ( 2 - ) or ( 35S ) methionine and immunoprecipitation demonstrated that ( 35S ) SO4 ( 2 - ) was efficiently incorporated into PAM proteins that have the noncatalytic exon A region following the monooxygenase domain ( PAM-1 and PAM-4 ) and into a soluble bifunctional PAM protein ( PAM-3 ) .
	manualset3
107677	9	402830	5	NULL	NULL	0	NULL	PAM-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic labeling with ( 35S ) SO4 ( 2 - ) or ( 35S ) methionine and immunoprecipitation demonstrated that ( 35S ) SO4 ( 2 - ) was efficiently incorporated into PAM proteins that have the noncatalytic exon A region following the monooxygenase domain ( PAM-1 and PAM-4 ) and into a soluble bifunctional PAM protein ( PAM-3 ) .
	manualset3
107678	10	402830	5	NULL	NULL	0	NULL	PAM-4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic labeling with ( 35S ) SO4 ( 2 - ) or ( 35S ) methionine and immunoprecipitation demonstrated that ( 35S ) SO4 ( 2 - ) was efficiently incorporated into PAM proteins that have the noncatalytic exon A region following the monooxygenase domain ( PAM-1 and PAM-4 ) and into a soluble bifunctional PAM protein ( PAM-3 ) .
	manualset3
107679	11	402830	5	NULL	NULL	0	NULL	soluble bifunctional PAM protein ( PAM-3 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic labeling with ( 35S ) SO4 ( 2 - ) or ( 35S ) methionine and immunoprecipitation demonstrated that ( 35S ) SO4 ( 2 - ) was efficiently incorporated into PAM proteins that have the noncatalytic exon A region following the monooxygenase domain ( PAM-1 and PAM-4 ) and into a soluble bifunctional PAM protein ( PAM-3 ) .
	manualset3
108093	1	402831	5	NULL	NULL	0	NULL	Metabolic liberation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic liberation of cyanide has been suggested to be responsible for the toxicity of ACN .
	manualset3
108094	2	402831	5	NULL	NULL	0	NULL	cyanide	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic liberation of cyanide has been suggested to be responsible for the toxicity of ACN .
	manualset3
108095	3	402831	5	NULL	NULL	0	NULL	toxicity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic liberation of cyanide has been suggested to be responsible for the toxicity of ACN .
	manualset3
108096	4	402831	5	NULL	NULL	0	NULL	ACN	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic liberation of cyanide has been suggested to be responsible for the toxicity of ACN .
	manualset3
108097	1	402832	5	NULL	NULL	0	NULL	Metabolic rate	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic rate , respiratory gas exchange , and nonprotein substrate oxidation were similar in both groups .
	manualset3
108098	2	402832	5	NULL	NULL	0	NULL	respiratory gas exchange	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic rate , respiratory gas exchange , and nonprotein substrate oxidation were similar in both groups .
	manualset3
108099	3	402832	5	NULL	NULL	0	NULL	nonprotein substrate oxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic rate , respiratory gas exchange , and nonprotein substrate oxidation were similar in both groups .
	manualset3
108100	4	402832	5	NULL	NULL	0	NULL	groups 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic rate , respiratory gas exchange , and nonprotein substrate oxidation were similar in both groups .
	manualset3
108103	1	402833	5	NULL	NULL	0	NULL	Metabolic response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic response to MMS-mediated DNA damage in Saccharomyces cerevisiae is dependent on the glucose concentration in the medium .
	manualset3
108104	2	402833	5	NULL	NULL	0	NULL	MMS-mediated DNA damage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic response to MMS-mediated DNA damage in Saccharomyces cerevisiae is dependent on the glucose concentration in the medium .
	manualset3
108105	3	402833	5	NULL	NULL	0	NULL	Saccharomyces cerevisiae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic response to MMS-mediated DNA damage in Saccharomyces cerevisiae is dependent on the glucose concentration in the medium .
	manualset3
108106	4	402833	5	NULL	NULL	0	NULL	glucose concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic response to MMS-mediated DNA damage in Saccharomyces cerevisiae is dependent on the glucose concentration in the medium .
	manualset3
108107	5	402833	5	NULL	NULL	0	NULL	medium 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic response to MMS-mediated DNA damage in Saccharomyces cerevisiae is dependent on the glucose concentration in the medium .
	manualset3
108108	1	402834	5	NULL	NULL	0	NULL	Metabolic studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic studies established that exogenously administered GM1 -- either embedded in liposomes or as a pure glycolipid dispersion -- led to the production of several products , including ceramide .
	manualset3
108109	2	402834	5	NULL	NULL	0	NULL	exogenously administered GM1	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic studies established that exogenously administered GM1 -- either embedded in liposomes or as a pure glycolipid dispersion -- led to the production of several products , including ceramide .
	manualset3
108110	3	402834	5	NULL	NULL	NULL	NULL	liposomes 	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Metabolic studies established that exogenously administered GM1 -- either embedded in liposomes or as a pure glycolipid dispersion -- led to the production of several products , including ceramide .
	manualset3
108111	4	402834	5	NULL	NULL	0	NULL	pure glycolipid dispersion	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic studies established that exogenously administered GM1 -- either embedded in liposomes or as a pure glycolipid dispersion -- led to the production of several products , including ceramide .
	manualset3
108112	5	402834	5	NULL	NULL	0	NULL	production 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic studies established that exogenously administered GM1 -- either embedded in liposomes or as a pure glycolipid dispersion -- led to the production of several products , including ceramide .
	manualset3
108113	6	402834	5	NULL	NULL	0	NULL	several products	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic studies established that exogenously administered GM1 -- either embedded in liposomes or as a pure glycolipid dispersion -- led to the production of several products , including ceramide .
	manualset3
108114	7	402834	5	NULL	NULL	0	NULL	ceramide	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic studies established that exogenously administered GM1 -- either embedded in liposomes or as a pure glycolipid dispersion -- led to the production of several products , including ceramide .
	manualset3
108115	1	402835	5	NULL	NULL	0	NULL	Metabolism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolism of 14C-naphthalene was studied in aerobic and anaerobic marine sediments from the Mumbai coast , India using a continuous flow-through system for 5 weeks .
	manualset3
108116	2	402835	5	NULL	NULL	0	NULL	14C-naphthalene	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolism of 14C-naphthalene was studied in aerobic and anaerobic marine sediments from the Mumbai coast , India using a continuous flow-through system for 5 weeks .
	manualset3
108117	3	402835	5	NULL	NULL	0	NULL	aerobic marine sediments	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolism of 14C-naphthalene was studied in aerobic and anaerobic marine sediments from the Mumbai coast , India using a continuous flow-through system for 5 weeks .
	manualset3
108118	4	402835	5	NULL	NULL	0	NULL	anaerobic marine sediments	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolism of 14C-naphthalene was studied in aerobic and anaerobic marine sediments from the Mumbai coast , India using a continuous flow-through system for 5 weeks .
	manualset3
108119	5	402835	5	NULL	NULL	NULL	NULL	Mumbai coast , India	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Metabolism of 14C-naphthalene was studied in aerobic and anaerobic marine sediments from the Mumbai coast , India using a continuous flow-through system for 5 weeks .
	manualset3
108120	6	402835	5	NULL	NULL	NULL	NULL	continuous flow-through system	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Metabolism of 14C-naphthalene was studied in aerobic and anaerobic marine sediments from the Mumbai coast , India using a continuous flow-through system for 5 weeks .
	manualset3
108121	7	402835	5	NULL	NULL	0	NULL	5 weeks 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolism of 14C-naphthalene was studied in aerobic and anaerobic marine sediments from the Mumbai coast , India using a continuous flow-through system for 5 weeks .
	manualset3
108122	1	402836	5	NULL	NULL	0	NULL	herpes simplex virus type 1 clones	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A broad variety of herpes simplex virus type 1 clones was selected under a single round of high-dose selection with brivudin .
	manualset3
108123	2	402836	5	NULL	NULL	0	NULL	high-dose selection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A broad variety of herpes simplex virus type 1 clones was selected under a single round of high-dose selection with brivudin .
	manualset3
108124	3	402836	5	NULL	NULL	0	NULL	brivudin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A broad variety of herpes simplex virus type 1 clones was selected under a single round of high-dose selection with brivudin .
	manualset3
108125	1	402837	5	NULL	NULL	0	NULL	Metabolism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolism of DDT in different tissues of young rats .
	manualset3
108126	2	402837	5	NULL	NULL	0	NULL	DDT	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolism of DDT in different tissues of young rats .
	manualset3
108127	3	402837	5	NULL	NULL	0	NULL	different tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolism of DDT in different tissues of young rats .
	manualset3
108128	4	402837	5	NULL	NULL	0	NULL	young rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolism of DDT in different tissues of young rats .
	manualset3
108129	1	402838	5	NULL	NULL	0	NULL	Metabolism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolism of prostaglandin E in dog kidneys .
	manualset3
108130	2	402838	5	NULL	NULL	0	NULL	prostaglandin E	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolism of prostaglandin E in dog kidneys .
	manualset3
108131	3	402838	5	NULL	NULL	0	NULL	dog kidneys	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolism of prostaglandin E in dog kidneys .
	manualset3
108132	1	402839	5	NULL	NULL	0	NULL	Metabolism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolism of the quinones by NQO1 revealed that , in general , compounds with electron-withdrawing groups at the indole 3-position were among the best substrates , and that groups larger than methyl at N-1 are clearly tolerated .
	manualset3
108133	2	402839	5	NULL	NULL	0	NULL	quinones 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolism of the quinones by NQO1 revealed that , in general , compounds with electron-withdrawing groups at the indole 3-position were among the best substrates , and that groups larger than methyl at N-1 are clearly tolerated .
	manualset3
108134	3	402839	5	NULL	NULL	0	NULL	NQO1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolism of the quinones by NQO1 revealed that , in general , compounds with electron-withdrawing groups at the indole 3-position were among the best substrates , and that groups larger than methyl at N-1 are clearly tolerated .
	manualset3
108135	4	402839	5	NULL	NULL	NULL	NULL	 compounds with electron-withdrawing groups at the indole 3-position	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Metabolism of the quinones by NQO1 revealed that , in general , compounds with electron-withdrawing groups at the indole 3-position were among the best substrates , and that groups larger than methyl at N-1 are clearly tolerated .
	manualset3
108138	5	402839	5	NULL	NULL	0	NULL	best substrates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolism of the quinones by NQO1 revealed that , in general , compounds with electron-withdrawing groups at the indole 3-position were among the best substrates , and that groups larger than methyl at N-1 are clearly tolerated .
	manualset3
108139	6	402839	5	NULL	NULL	0	NULL	groups larger than methyl at N-1	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolism of the quinones by NQO1 revealed that , in general , compounds with electron-withdrawing groups at the indole 3-position were among the best substrates , and that groups larger than methyl at N-1 are clearly tolerated .
	manualset3
108140	1	402840	5	NULL	NULL	0	NULL	Metabolite excretions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolite excretions were found to be significantly ( p & lt ; 0.0001 ) higher for both plateletpheresis techniques compared to plasmapheresis and controls .
	manualset3
108141	2	402840	5	NULL	NULL	0	NULL	p & lt ; 0.0001 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolite excretions were found to be significantly ( p & lt ; 0.0001 ) higher for both plateletpheresis techniques compared to plasmapheresis and controls .
	manualset3
108142	3	402840	5	NULL	NULL	0	NULL	plateletpheresis techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolite excretions were found to be significantly ( p & lt ; 0.0001 ) higher for both plateletpheresis techniques compared to plasmapheresis and controls .
	manualset3
108143	4	402840	5	NULL	NULL	0	NULL	plasmapheresis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolite excretions were found to be significantly ( p & lt ; 0.0001 ) higher for both plateletpheresis techniques compared to plasmapheresis and controls .
	manualset3
108144	5	402840	5	NULL	NULL	0	NULL	controls 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolite excretions were found to be significantly ( p & lt ; 0.0001 ) higher for both plateletpheresis techniques compared to plasmapheresis and controls .
	manualset3
108145	1	402841	5	NULL	NULL	0	NULL	Metabolite profile analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolite profile analysis : from raw data to regression and classification .
	manualset3
108146	2	402841	5	NULL	NULL	0	NULL	raw data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolite profile analysis : from raw data to regression and classification .
	manualset3
108147	3	402841	5	NULL	NULL	0	NULL	regression 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolite profile analysis : from raw data to regression and classification .
	manualset3
108148	4	402841	5	NULL	NULL	0	NULL	classification 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolite profile analysis : from raw data to regression and classification .
	manualset3
108149	1	402842	5	NULL	NULL	0	NULL	Metabolites 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolites in urine of rat were examined with chromatography .
	manualset3
108150	2	402842	5	NULL	NULL	NULL	NULL	urine 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Metabolites in urine of rat were examined with chromatography .
	manualset3
108151	3	402842	5	NULL	NULL	0	NULL	rat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolites in urine of rat were examined with chromatography .
	manualset3
108152	4	402842	5	NULL	NULL	0	NULL	chromatography 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolites in urine of rat were examined with chromatography .
	manualset3
108153	1	402843	5	NULL	NULL	0	NULL	Metacycline 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Metacycline was shown in in vitro experiments to inhibit gelatinase B. The combination of peroral D-penicillamine plus metacycline was evaluated in a double-blind placebo-controlled way in two groups of 10 patients suffering from secondary progressive multiple sclerosis .
	manualset3
108154	2	402843	5	NULL	NULL	0	NULL	in vitro experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Metacycline was shown in in vitro experiments to inhibit gelatinase B. The combination of peroral D-penicillamine plus metacycline was evaluated in a double-blind placebo-controlled way in two groups of 10 patients suffering from secondary progressive multiple sclerosis .
	manualset3
108155	3	402843	5	NULL	NULL	0	NULL	gelatinase B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Metacycline was shown in in vitro experiments to inhibit gelatinase B. The combination of peroral D-penicillamine plus metacycline was evaluated in a double-blind placebo-controlled way in two groups of 10 patients suffering from secondary progressive multiple sclerosis .
	manualset3
108156	4	402843	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Metacycline was shown in in vitro experiments to inhibit gelatinase B. The combination of peroral D-penicillamine plus metacycline was evaluated in a double-blind placebo-controlled way in two groups of 10 patients suffering from secondary progressive multiple sclerosis .
	manualset3
108157	5	402843	5	NULL	NULL	0	NULL	peroral D-penicillamine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Metacycline was shown in in vitro experiments to inhibit gelatinase B. The combination of peroral D-penicillamine plus metacycline was evaluated in a double-blind placebo-controlled way in two groups of 10 patients suffering from secondary progressive multiple sclerosis .
	manualset3
108158	6	402843	5	NULL	NULL	0	NULL	metacycline 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Metacycline was shown in in vitro experiments to inhibit gelatinase B. The combination of peroral D-penicillamine plus metacycline was evaluated in a double-blind placebo-controlled way in two groups of 10 patients suffering from secondary progressive multiple sclerosis .
	manualset3
108159	7	402843	5	NULL	NULL	0	NULL	double-blind placebo-controlled way	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Metacycline was shown in in vitro experiments to inhibit gelatinase B. The combination of peroral D-penicillamine plus metacycline was evaluated in a double-blind placebo-controlled way in two groups of 10 patients suffering from secondary progressive multiple sclerosis .
	manualset3
108160	8	402843	5	NULL	NULL	NULL	NULL	two groups of 10 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Metacycline was shown in in vitro experiments to inhibit gelatinase B. The combination of peroral D-penicillamine plus metacycline was evaluated in a double-blind placebo-controlled way in two groups of 10 patients suffering from secondary progressive multiple sclerosis .
	manualset3
108161	9	402843	5	NULL	NULL	0	NULL	secondary progressive multiple sclerosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Metacycline was shown in in vitro experiments to inhibit gelatinase B. The combination of peroral D-penicillamine plus metacycline was evaluated in a double-blind placebo-controlled way in two groups of 10 patients suffering from secondary progressive multiple sclerosis .
	manualset3
108162	1	402844	5	NULL	NULL	0	NULL	Metal-based nanoparticles	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Metal-based nanoparticles in soil : Fate , behavior , and effects on soil invertebrates .
	manualset3
108163	2	402844	5	NULL	NULL	0	NULL	soil 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Metal-based nanoparticles in soil : Fate , behavior , and effects on soil invertebrates .
	manualset3
108165	3	402844	5	NULL	NULL	0	NULL	Fate 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Metal-based nanoparticles in soil : Fate , behavior , and effects on soil invertebrates .
	manualset3
108166	4	402844	5	NULL	NULL	0	NULL	behavior 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Metal-based nanoparticles in soil : Fate , behavior , and effects on soil invertebrates .
	manualset3
108167	5	402844	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Metal-based nanoparticles in soil : Fate , behavior , and effects on soil invertebrates .
	manualset3
108168	6	402844	5	NULL	NULL	0	NULL	soil invertebrates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Metal-based nanoparticles in soil : Fate , behavior , and effects on soil invertebrates .
	manualset3
108169	1	402845	5	NULL	NULL	0	NULL	Metal-independent decomposition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Metal-independent decomposition of hydroperoxides by halogenated quinones : detection and identification of a quinone ketoxy radical .
	manualset3
108170	2	402845	5	NULL	NULL	0	NULL	hydroperoxides 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Metal-independent decomposition of hydroperoxides by halogenated quinones : detection and identification of a quinone ketoxy radical .
	manualset3
108171	3	402845	5	NULL	NULL	0	NULL	halogenated quinones	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Metal-independent decomposition of hydroperoxides by halogenated quinones : detection and identification of a quinone ketoxy radical .
	manualset3
108172	4	402845	5	NULL	NULL	NULL	NULL	detection 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Metal-independent decomposition of hydroperoxides by halogenated quinones : detection and identification of a quinone ketoxy radical .
	manualset3
108173	5	402845	5	NULL	NULL	NULL	NULL	identification 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Metal-independent decomposition of hydroperoxides by halogenated quinones : detection and identification of a quinone ketoxy radical .
	manualset3
108174	6	402845	5	NULL	NULL	0	NULL	quinone ketoxy radical 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Metal-independent decomposition of hydroperoxides by halogenated quinones : detection and identification of a quinone ketoxy radical .
	manualset3
108175	1	402846	5	NULL	NULL	0	NULL	Behavior 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Behavior of alpha-1-fetoprotein in premature infants ) .
	manualset3
108176	2	402846	5	NULL	NULL	0	NULL	alpha-1-fetoprotein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Behavior of alpha-1-fetoprotein in premature infants ) .
	manualset3
108177	3	402846	5	NULL	NULL	0	NULL	premature infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Behavior of alpha-1-fetoprotein in premature infants ) .
	manualset3
108178	1	402847	5	NULL	NULL	0	NULL	broadband detection performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A broadband detection performance of a circular microphone array has been degenerated by discrete noise interference .
	manualset3
108179	2	402847	5	NULL	NULL	0	NULL	circular microphone array	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A broadband detection performance of a circular microphone array has been degenerated by discrete noise interference .
	manualset3
108180	3	402847	5	NULL	NULL	0	NULL	discrete noise interference 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A broadband detection performance of a circular microphone array has been degenerated by discrete noise interference .
	manualset3
108181	1	402848	5	NULL	NULL	0	NULL	Metal-ligand bifunctional activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Metal-ligand bifunctional activation and transfer of N-H bonds .
	manualset3
108182	1	402848	5	NULL	NULL	0	NULL	Metal-ligand bifunctional activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Metal-ligand bifunctional activation and transfer of N-H bonds .
	manualset3
108183	2	402848	5	NULL	NULL	NULL	NULL	N-H bonds	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Metal-ligand bifunctional activation and transfer of N-H bonds .
	manualset3
108184	1	402849	5	NULL	NULL	0	NULL	Metalloproteases 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Metalloproteases of the M13 subfamily , comprising namely neprylisin ( NEP ) and endothelin-converting enzyme ( ECE ) , are involved in the metabolism of various neuronal and hormonal peptides , and inhibitors thereof have already led to therapeutically useful agents .
	manualset3
108185	2	402849	5	NULL	NULL	0	NULL	M13 subfamily	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Metalloproteases of the M13 subfamily , comprising namely neprylisin ( NEP ) and endothelin-converting enzyme ( ECE ) , are involved in the metabolism of various neuronal and hormonal peptides , and inhibitors thereof have already led to therapeutically useful agents .
	manualset3
108186	3	402849	5	NULL	NULL	0	NULL	neprylisin ( NEP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Metalloproteases of the M13 subfamily , comprising namely neprylisin ( NEP ) and endothelin-converting enzyme ( ECE ) , are involved in the metabolism of various neuronal and hormonal peptides , and inhibitors thereof have already led to therapeutically useful agents .
	manualset3
108187	4	402849	5	NULL	NULL	0	NULL	endothelin-converting enzyme ( ECE )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Metalloproteases of the M13 subfamily , comprising namely neprylisin ( NEP ) and endothelin-converting enzyme ( ECE ) , are involved in the metabolism of various neuronal and hormonal peptides , and inhibitors thereof have already led to therapeutically useful agents .
	manualset3
108188	5	402849	5	NULL	NULL	0	NULL	metabolism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Metalloproteases of the M13 subfamily , comprising namely neprylisin ( NEP ) and endothelin-converting enzyme ( ECE ) , are involved in the metabolism of various neuronal and hormonal peptides , and inhibitors thereof have already led to therapeutically useful agents .
	manualset3
108189	6	402849	5	NULL	NULL	0	NULL	neuronal peptides	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Metalloproteases of the M13 subfamily , comprising namely neprylisin ( NEP ) and endothelin-converting enzyme ( ECE ) , are involved in the metabolism of various neuronal and hormonal peptides , and inhibitors thereof have already led to therapeutically useful agents .
	manualset3
108190	7	402849	5	NULL	NULL	0	NULL	hormonal peptides	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Metalloproteases of the M13 subfamily , comprising namely neprylisin ( NEP ) and endothelin-converting enzyme ( ECE ) , are involved in the metabolism of various neuronal and hormonal peptides , and inhibitors thereof have already led to therapeutically useful agents .
	manualset3
108191	8	402849	5	NULL	NULL	0	NULL	inhibitors 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Metalloproteases of the M13 subfamily , comprising namely neprylisin ( NEP ) and endothelin-converting enzyme ( ECE ) , are involved in the metabolism of various neuronal and hormonal peptides , and inhibitors thereof have already led to therapeutically useful agents .
	manualset3
108192	9	402849	5	NULL	NULL	0	NULL	therapeutically useful agents	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Metalloproteases of the M13 subfamily , comprising namely neprylisin ( NEP ) and endothelin-converting enzyme ( ECE ) , are involved in the metabolism of various neuronal and hormonal peptides , and inhibitors thereof have already led to therapeutically useful agents .
	manualset3
108193	1	402850	5	NULL	NULL	0	NULL	Metalloproteinase-9	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Metalloproteinase-9 is increased after toluene diisocyanate exposure in the induced sputum from patients with toluene diisocyanate-induced asthma .
	manualset3
108194	2	402850	5	NULL	NULL	0	NULL	toluene diisocyanate exposure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Metalloproteinase-9 is increased after toluene diisocyanate exposure in the induced sputum from patients with toluene diisocyanate-induced asthma .
	manualset3
108195	3	402850	5	NULL	NULL	0	NULL	induced sputum	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Metalloproteinase-9 is increased after toluene diisocyanate exposure in the induced sputum from patients with toluene diisocyanate-induced asthma .
	manualset3
108196	4	402850	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Metalloproteinase-9 is increased after toluene diisocyanate exposure in the induced sputum from patients with toluene diisocyanate-induced asthma .
	manualset3
108197	5	402850	5	NULL	NULL	0	NULL	toluene diisocyanate-induced asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Metalloproteinase-9 is increased after toluene diisocyanate exposure in the induced sputum from patients with toluene diisocyanate-induced asthma .
	manualset3
108198	1	402851	5	NULL	NULL	0	NULL	Metalloregulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Metalloregulation of FRE1 and FRE2 homologs in Saccharomyces cerevisiae .
	manualset3
108199	2	402851	5	NULL	NULL	0	NULL	FRE1 homologs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Metalloregulation of FRE1 and FRE2 homologs in Saccharomyces cerevisiae .
	manualset3
108200	3	402851	5	NULL	NULL	0	NULL	FRE2 homologs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Metalloregulation of FRE1 and FRE2 homologs in Saccharomyces cerevisiae .
	manualset3
108201	4	402851	5	NULL	NULL	0	NULL	Saccharomyces cerevisiae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Metalloregulation of FRE1 and FRE2 homologs in Saccharomyces cerevisiae .
	manualset3
108202	1	402852	5	NULL	NULL	0	NULL	Metallothioneins ( MTs )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Metallothioneins ( MTs ) are known as heat-stable proteins and are able to be precipitated at 100 degrees C for 2 min .
	manualset3
108203	2	402852	5	NULL	NULL	0	NULL	heat-stable proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Metallothioneins ( MTs ) are known as heat-stable proteins and are able to be precipitated at 100 degrees C for 2 min .
	manualset3
108204	3	402852	5	NULL	NULL	0	NULL	100 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Metallothioneins ( MTs ) are known as heat-stable proteins and are able to be precipitated at 100 degrees C for 2 min .
	manualset3
108205	4	402852	5	NULL	NULL	0	NULL	2 min	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Metallothioneins ( MTs ) are known as heat-stable proteins and are able to be precipitated at 100 degrees C for 2 min .
	manualset3
108206	1	402853	5	NULL	NULL	0	NULL	Metamine ( triethanolamine trinitrate biphosphate )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Metamine ( triethanolamine trinitrate biphosphate ) in angina pectoris .
	manualset3
108207	2	402853	5	NULL	NULL	0	NULL	angina pectoris	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Metamine ( triethanolamine trinitrate biphosphate ) in angina pectoris .
	manualset3
108208	1	402854	5	NULL	NULL	0	NULL	partners 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Metaphorically , the partners negotiate the conditions of trade , the outcome of which will determine the net benefit to each partner .
	manualset3
108209	2	402854	5	NULL	NULL	0	NULL	conditions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Metaphorically , the partners negotiate the conditions of trade , the outcome of which will determine the net benefit to each partner .
	manualset3
108210	3	402854	5	NULL	NULL	0	NULL	trade 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Metaphorically , the partners negotiate the conditions of trade , the outcome of which will determine the net benefit to each partner .
	manualset3
108211	4	402854	5	NULL	NULL	0	NULL	outcome 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Metaphorically , the partners negotiate the conditions of trade , the outcome of which will determine the net benefit to each partner .
	manualset3
108212	5	402854	5	NULL	NULL	NULL	NULL	net benefit 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Metaphorically , the partners negotiate the conditions of trade , the outcome of which will determine the net benefit to each partner .
	manualset3
108213	6	402854	5	NULL	NULL	0	NULL	partner 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Metaphorically , the partners negotiate the conditions of trade , the outcome of which will determine the net benefit to each partner .
	manualset3
108214	1	402855	5	NULL	NULL	0	NULL	Metastable fragmentation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Metastable fragmentation of neon dimer ions has been investigated by measuring and analyzing high resolution kinetic energy release distributions .
	manualset3
108215	2	402855	5	NULL	NULL	0	NULL	neon dimer ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Metastable fragmentation of neon dimer ions has been investigated by measuring and analyzing high resolution kinetic energy release distributions .
	manualset3
108216	3	402855	5	NULL	NULL	0	NULL	high resolution kinetic energy release distributions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Metastable fragmentation of neon dimer ions has been investigated by measuring and analyzing high resolution kinetic energy release distributions .
	manualset3
108217	1	402856	5	NULL	NULL	0	NULL	Metastatic tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Metastatic tumors of the stomach are rare .
	manualset3
108218	2	402856	5	NULL	NULL	0	NULL	stomach 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Metastatic tumors of the stomach are rare .
	manualset3
108219	1	402857	5	NULL	NULL	0	NULL	brother 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A brother of the index case was 36 years old and free of cardiac history and symptoms .
	manualset3
108220	2	402857	5	NULL	NULL	0	NULL	index case 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A brother of the index case was 36 years old and free of cardiac history and symptoms .
	manualset3
108221	3	402857	5	NULL	NULL	0	NULL	36 years old 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A brother of the index case was 36 years old and free of cardiac history and symptoms .
	manualset3
108222	4	402857	5	NULL	NULL	0	NULL	free of cardiac history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A brother of the index case was 36 years old and free of cardiac history and symptoms .
	manualset3
108223	5	402857	5	NULL	NULL	0	NULL	symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A brother of the index case was 36 years old and free of cardiac history and symptoms .
	manualset3
108224	1	402858	5	NULL	NULL	0	NULL	Metastatic variants	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Metastatic variants of the B16 melanoma displaying high experimental metastatic potential have been shown to express high levels of a 72 , 000-dalton glycoprotein ( Met-72 ) on their cell surface ( Kimura AK , Xiang J : J Nat Can Inst 76 : 1247 -1253 , 1986 ) .
	manualset3
108225	2	402858	5	NULL	NULL	0	NULL	B16 melanoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Metastatic variants of the B16 melanoma displaying high experimental metastatic potential have been shown to express high levels of a 72 , 000-dalton glycoprotein ( Met-72 ) on their cell surface ( Kimura AK , Xiang J : J Nat Can Inst 76 : 1247 -1253 , 1986 ) .
	manualset3
108226	3	402858	5	NULL	NULL	0	NULL	high experimental metastatic potential	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Metastatic variants of the B16 melanoma displaying high experimental metastatic potential have been shown to express high levels of a 72 , 000-dalton glycoprotein ( Met-72 ) on their cell surface ( Kimura AK , Xiang J : J Nat Can Inst 76 : 1247 -1253 , 1986 ) .
	manualset3
108227	4	402858	5	NULL	NULL	0	NULL	high levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Metastatic variants of the B16 melanoma displaying high experimental metastatic potential have been shown to express high levels of a 72 , 000-dalton glycoprotein ( Met-72 ) on their cell surface ( Kimura AK , Xiang J : J Nat Can Inst 76 : 1247 -1253 , 1986 ) .
	manualset3
108228	5	402858	5	NULL	NULL	0	NULL	72 , 000-dalton glycoprotein ( Met-72 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Metastatic variants of the B16 melanoma displaying high experimental metastatic potential have been shown to express high levels of a 72 , 000-dalton glycoprotein ( Met-72 ) on their cell surface ( Kimura AK , Xiang J : J Nat Can Inst 76 : 1247 -1253 , 1986 ) .
	manualset3
108229	6	402858	5	NULL	NULL	0	NULL	cell surface	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Metastatic variants of the B16 melanoma displaying high experimental metastatic potential have been shown to express high levels of a 72 , 000-dalton glycoprotein ( Met-72 ) on their cell surface ( Kimura AK , Xiang J : J Nat Can Inst 76 : 1247 -1253 , 1986 ) .
	manualset3
108230	7	402858	5	NULL	NULL	0	NULL	Kimura AK	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Metastatic variants of the B16 melanoma displaying high experimental metastatic potential have been shown to express high levels of a 72 , 000-dalton glycoprotein ( Met-72 ) on their cell surface ( Kimura AK , Xiang J : J Nat Can Inst 76 : 1247 -1253 , 1986 ) .
	manualset3
108231	8	402858	5	NULL	NULL	0	NULL	Xiang J	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Metastatic variants of the B16 melanoma displaying high experimental metastatic potential have been shown to express high levels of a 72 , 000-dalton glycoprotein ( Met-72 ) on their cell surface ( Kimura AK , Xiang J : J Nat Can Inst 76 : 1247 -1253 , 1986 ) .
	manualset3
108232	9	402858	5	NULL	NULL	0	NULL	J Nat Can Inst 76 : 1247 -1253 , 1986	Citation												NULL		0	NULL	NULL	NULL	NULL	NULL	Metastatic variants of the B16 melanoma displaying high experimental metastatic potential have been shown to express high levels of a 72 , 000-dalton glycoprotein ( Met-72 ) on their cell surface ( Kimura AK , Xiang J : J Nat Can Inst 76 : 1247 -1253 , 1986 ) .
	manualset3
108233	1	402859	5	NULL	NULL	0	NULL	Metformin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Metformin does not increase energy expenditure of brown fat .
	manualset3
108234	2	402859	5	NULL	NULL	0	NULL	energy expenditure	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Metformin does not increase energy expenditure of brown fat .
	manualset3
108235	3	402859	5	NULL	NULL	0	NULL	brown fat	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Metformin does not increase energy expenditure of brown fat .
	manualset3
108236	1	402860	5	NULL	NULL	NULL	NULL	Methamphetamine dependence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Methamphetamine dependence presents a serious problem not only for patients but also for society .
	manualset3
108237	2	402860	5	NULL	NULL	0	NULL	serious problem 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Methamphetamine dependence presents a serious problem not only for patients but also for society .
	manualset3
108238	3	402860	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Methamphetamine dependence presents a serious problem not only for patients but also for society .
	manualset3
108239	4	402860	5	NULL	NULL	0	NULL	society 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Methamphetamine dependence presents a serious problem not only for patients but also for society .
	manualset3
108240	1	402861	5	NULL	NULL	0	NULL	Methanol extract consumption 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methanol extract consumption of Quercus infectoria significantly decreased plasma levels of TC , TG and LDL ( p & lt ; 0.001 ) .
	manualset3
108241	2	402861	5	NULL	NULL	0	NULL	Quercus infectoria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Methanol extract consumption of Quercus infectoria significantly decreased plasma levels of TC , TG and LDL ( p & lt ; 0.001 ) .
	manualset3
108242	3	402861	5	NULL	NULL	0	NULL	plasma levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methanol extract consumption of Quercus infectoria significantly decreased plasma levels of TC , TG and LDL ( p & lt ; 0.001 ) .
	manualset3
108243	4	402861	5	NULL	NULL	0	NULL	TC 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Methanol extract consumption of Quercus infectoria significantly decreased plasma levels of TC , TG and LDL ( p & lt ; 0.001 ) .
	manualset3
108244	5	402861	5	NULL	NULL	0	NULL	TG	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Methanol extract consumption of Quercus infectoria significantly decreased plasma levels of TC , TG and LDL ( p & lt ; 0.001 ) .
	manualset3
108245	6	402861	5	NULL	NULL	0	NULL	LDL 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Methanol extract consumption of Quercus infectoria significantly decreased plasma levels of TC , TG and LDL ( p & lt ; 0.001 ) .
	manualset3
108246	7	402861	5	NULL	NULL	0	NULL	p & lt ; 0.001 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Methanol extract consumption of Quercus infectoria significantly decreased plasma levels of TC , TG and LDL ( p & lt ; 0.001 ) .
	manualset3
108247	1	402862	5	NULL	NULL	0	NULL	Methicillin-resistant Staphylococcus aureus ( MRSA )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Methicillin-resistant Staphylococcus aureus ( MRSA ) is an important human pathogen and represents a growing public health burden due to the emergence and spread of epidemic strains , particularly within the hospital environment .
	manualset3
108248	2	402862	5	NULL	NULL	0	NULL	important human pathogen	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Methicillin-resistant Staphylococcus aureus ( MRSA ) is an important human pathogen and represents a growing public health burden due to the emergence and spread of epidemic strains , particularly within the hospital environment .
	manualset3
108249	3	402862	5	NULL	NULL	0	NULL	growing public health burden	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methicillin-resistant Staphylococcus aureus ( MRSA ) is an important human pathogen and represents a growing public health burden due to the emergence and spread of epidemic strains , particularly within the hospital environment .
	manualset3
108250	4	402862	5	NULL	NULL	0	NULL	epidemic strains 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Methicillin-resistant Staphylococcus aureus ( MRSA ) is an important human pathogen and represents a growing public health burden due to the emergence and spread of epidemic strains , particularly within the hospital environment .
	manualset3
108251	5	402862	5	NULL	NULL	0	NULL	hospital environment	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Methicillin-resistant Staphylococcus aureus ( MRSA ) is an important human pathogen and represents a growing public health burden due to the emergence and spread of epidemic strains , particularly within the hospital environment .
	manualset3
108252	1	402863	5	NULL	NULL	0	NULL	Methicillin-resistant Staphylococcus aureus ( MRSA )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Methicillin-resistant Staphylococcus aureus ( MRSA ) is the major global nosocomial infection and resistance to vancomycin is evident and may become common .
	manualset3
108253	2	402863	5	NULL	NULL	0	NULL	major global nosocomial infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Methicillin-resistant Staphylococcus aureus ( MRSA ) is the major global nosocomial infection and resistance to vancomycin is evident and may become common .
	manualset3
108254	3	402863	5	NULL	NULL	0	NULL	resistance to vancomycin	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Methicillin-resistant Staphylococcus aureus ( MRSA ) is the major global nosocomial infection and resistance to vancomycin is evident and may become common .
	manualset3
108255	1	402864	5	NULL	NULL	0	NULL	Method 2	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Method 2 was similar to Method 1 , but corrected for shortening of the long axis of the left ventricle .
	manualset3
108256	2	402864	5	NULL	NULL	0	NULL	Method 1	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Method 2 was similar to Method 1 , but corrected for shortening of the long axis of the left ventricle .
	manualset3
108257	3	402864	5	NULL	NULL	0	NULL	long axis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Method 2 was similar to Method 1 , but corrected for shortening of the long axis of the left ventricle .
	manualset3
108258	4	402864	5	NULL	NULL	0	NULL	left ventricle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Method 2 was similar to Method 1 , but corrected for shortening of the long axis of the left ventricle .
	manualset3
108259	1	402865	5	NULL	NULL	0	NULL	Method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Method : This is a longitudinal study of a community sample of 649 pregnant women who were assessed in early pregnancy ( 17.4 4.9 weeks ) , late pregnancy ( 30.6 2.7 weeks ) , and postpartum ( 4.2 2.1 weeks ) with the Edinburgh Postnatal Depression Scale ( EPDS ) .
	manualset3
108260	2	402865	5	NULL	NULL	0	NULL	longitudinal study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Method : This is a longitudinal study of a community sample of 649 pregnant women who were assessed in early pregnancy ( 17.4 4.9 weeks ) , late pregnancy ( 30.6 2.7 weeks ) , and postpartum ( 4.2 2.1 weeks ) with the Edinburgh Postnatal Depression Scale ( EPDS ) .
	manualset3
108261	3	402865	5	NULL	NULL	0	NULL	community sample	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Method : This is a longitudinal study of a community sample of 649 pregnant women who were assessed in early pregnancy ( 17.4 4.9 weeks ) , late pregnancy ( 30.6 2.7 weeks ) , and postpartum ( 4.2 2.1 weeks ) with the Edinburgh Postnatal Depression Scale ( EPDS ) .
	manualset3
108262	4	402865	5	NULL	NULL	0	NULL	 649 pregnant women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Method : This is a longitudinal study of a community sample of 649 pregnant women who were assessed in early pregnancy ( 17.4 4.9 weeks ) , late pregnancy ( 30.6 2.7 weeks ) , and postpartum ( 4.2 2.1 weeks ) with the Edinburgh Postnatal Depression Scale ( EPDS ) .
	manualset3
108263	5	402865	5	NULL	NULL	NULL	NULL	early pregnancy	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Method : This is a longitudinal study of a community sample of 649 pregnant women who were assessed in early pregnancy ( 17.4 4.9 weeks ) , late pregnancy ( 30.6 2.7 weeks ) , and postpartum ( 4.2 2.1 weeks ) with the Edinburgh Postnatal Depression Scale ( EPDS ) .
	manualset3
108264	6	402865	5	NULL	NULL	0	NULL	17.4 4.9 weeks 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Method : This is a longitudinal study of a community sample of 649 pregnant women who were assessed in early pregnancy ( 17.4 4.9 weeks ) , late pregnancy ( 30.6 2.7 weeks ) , and postpartum ( 4.2 2.1 weeks ) with the Edinburgh Postnatal Depression Scale ( EPDS ) .
	manualset3
108265	7	402865	5	NULL	NULL	0	NULL	late pregnancy	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Method : This is a longitudinal study of a community sample of 649 pregnant women who were assessed in early pregnancy ( 17.4 4.9 weeks ) , late pregnancy ( 30.6 2.7 weeks ) , and postpartum ( 4.2 2.1 weeks ) with the Edinburgh Postnatal Depression Scale ( EPDS ) .
	manualset3
108266	8	402865	5	NULL	NULL	0	NULL	30.6 2.7 weeks 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Method : This is a longitudinal study of a community sample of 649 pregnant women who were assessed in early pregnancy ( 17.4 4.9 weeks ) , late pregnancy ( 30.6 2.7 weeks ) , and postpartum ( 4.2 2.1 weeks ) with the Edinburgh Postnatal Depression Scale ( EPDS ) .
	manualset3
108267	9	402865	5	NULL	NULL	0	NULL	postpartum 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Method : This is a longitudinal study of a community sample of 649 pregnant women who were assessed in early pregnancy ( 17.4 4.9 weeks ) , late pregnancy ( 30.6 2.7 weeks ) , and postpartum ( 4.2 2.1 weeks ) with the Edinburgh Postnatal Depression Scale ( EPDS ) .
	manualset3
108268	10	402865	5	NULL	NULL	0	NULL	 4.2 2.1 weeks	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Method : This is a longitudinal study of a community sample of 649 pregnant women who were assessed in early pregnancy ( 17.4 4.9 weeks ) , late pregnancy ( 30.6 2.7 weeks ) , and postpartum ( 4.2 2.1 weeks ) with the Edinburgh Postnatal Depression Scale ( EPDS ) .
	manualset3
108269	11	402865	5	NULL	NULL	0	NULL	Edinburgh Postnatal Depression Scale ( EPDS )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Method : This is a longitudinal study of a community sample of 649 pregnant women who were assessed in early pregnancy ( 17.4 4.9 weeks ) , late pregnancy ( 30.6 2.7 weeks ) , and postpartum ( 4.2 2.1 weeks ) with the Edinburgh Postnatal Depression Scale ( EPDS ) .
	manualset3
108270	1	402866	5	NULL	NULL	0	NULL	buildup requirement	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A buildup requirement again debates the question of alternative to amalgam .
	manualset3
108271	2	402866	5	NULL	NULL	0	NULL	question 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A buildup requirement again debates the question of alternative to amalgam .
	manualset3
108272	3	402866	5	NULL	NULL	0	NULL	amalgam 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A buildup requirement again debates the question of alternative to amalgam .
	manualset3
108273	1	402867	5	NULL	NULL	0	NULL	Method I	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Method I required total lipid extraction , separation of FFA by thin-layer chromatography , methylation , and gas-liquid chromatographic analysis of the fatty acid ( FA ) methyl esters .
	manualset3
108274	2	402867	5	NULL	NULL	0	NULL	total lipid extraction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Method I required total lipid extraction , separation of FFA by thin-layer chromatography , methylation , and gas-liquid chromatographic analysis of the fatty acid ( FA ) methyl esters .
	manualset3
108275	3	402867	5	NULL	NULL	0	NULL	separation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Method I required total lipid extraction , separation of FFA by thin-layer chromatography , methylation , and gas-liquid chromatographic analysis of the fatty acid ( FA ) methyl esters .
	manualset3
108276	4	402867	5	NULL	NULL	0	NULL	FFA 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Method I required total lipid extraction , separation of FFA by thin-layer chromatography , methylation , and gas-liquid chromatographic analysis of the fatty acid ( FA ) methyl esters .
	manualset3
108277	5	402867	5	NULL	NULL	0	NULL	thin-layer chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Method I required total lipid extraction , separation of FFA by thin-layer chromatography , methylation , and gas-liquid chromatographic analysis of the fatty acid ( FA ) methyl esters .
	manualset3
108278	6	402867	5	NULL	NULL	0	NULL	methylation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Method I required total lipid extraction , separation of FFA by thin-layer chromatography , methylation , and gas-liquid chromatographic analysis of the fatty acid ( FA ) methyl esters .
	manualset3
108279	7	402867	5	NULL	NULL	0	NULL	gas-liquid chromatographic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Method I required total lipid extraction , separation of FFA by thin-layer chromatography , methylation , and gas-liquid chromatographic analysis of the fatty acid ( FA ) methyl esters .
	manualset3
108280	8	402867	5	NULL	NULL	0	NULL	fatty acid ( FA ) methyl esters	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Method I required total lipid extraction , separation of FFA by thin-layer chromatography , methylation , and gas-liquid chromatographic analysis of the fatty acid ( FA ) methyl esters .
	manualset3
108281	1	402868	5	NULL	NULL	0	NULL	Methodological quality	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Methodological quality Two independent reviewers assessed the methodological quality of retrieved papers using the corresponding checklist from the System for the Unified Management , Assessment and Review of Information ( SUMARI ) package .
	manualset3
108282	2	402868	5	NULL	NULL	0	NULL	Two independent reviewers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Methodological quality Two independent reviewers assessed the methodological quality of retrieved papers using the corresponding checklist from the System for the Unified Management , Assessment and Review of Information ( SUMARI ) package .
	manualset3
108283	3	402868	5	NULL	NULL	NULL	NULL	methodological quality	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Methodological quality Two independent reviewers assessed the methodological quality of retrieved papers using the corresponding checklist from the System for the Unified Management , Assessment and Review of Information ( SUMARI ) package .
	manualset3
108284	4	402868	5	NULL	NULL	0	NULL	retrieved papers	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Methodological quality Two independent reviewers assessed the methodological quality of retrieved papers using the corresponding checklist from the System for the Unified Management , Assessment and Review of Information ( SUMARI ) package .
	manualset3
108285	5	402868	5	NULL	NULL	0	NULL	checklist 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methodological quality Two independent reviewers assessed the methodological quality of retrieved papers using the corresponding checklist from the System for the Unified Management , Assessment and Review of Information ( SUMARI ) package .
	manualset3
108286	6	402868	5	NULL	NULL	0	NULL	System for the Unified Management , Assessment and Review of Information ( SUMARI ) package	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Methodological quality Two independent reviewers assessed the methodological quality of retrieved papers using the corresponding checklist from the System for the Unified Management , Assessment and Review of Information ( SUMARI ) package .
	manualset3
108287	1	402869	5	NULL	NULL	0	NULL	Methods 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods , such as color naming and hue scaling , aim at describing color in terms of the relative amount of the component hues .
	manualset3
108288	2	402869	5	NULL	NULL	NULL	NULL	color naming	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Methods , such as color naming and hue scaling , aim at describing color in terms of the relative amount of the component hues .
	manualset3
108289	3	402869	5	NULL	NULL	0	NULL	hue scaling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods , such as color naming and hue scaling , aim at describing color in terms of the relative amount of the component hues .
	manualset3
108290	4	402869	5	NULL	NULL	0	NULL	color 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods , such as color naming and hue scaling , aim at describing color in terms of the relative amount of the component hues .
	manualset3
108291	5	402869	5	NULL	NULL	0	NULL	relative amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods , such as color naming and hue scaling , aim at describing color in terms of the relative amount of the component hues .
	manualset3
108292	6	402869	5	NULL	NULL	0	NULL	component hues	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods , such as color naming and hue scaling , aim at describing color in terms of the relative amount of the component hues .
	manualset3
108293	1	402870	5	NULL	NULL	0	NULL	Methods 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : A Varian TrueBeam linac with a maximum photon energy of 15 MV was installed in asmaller , preexisting vault .
	manualset3
108294	2	402870	5	NULL	NULL	NULL	NULL	Varian TrueBeam linac	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Methods : A Varian TrueBeam linac with a maximum photon energy of 15 MV was installed in asmaller , preexisting vault .
	manualset3
108295	3	402870	5	NULL	NULL	0	NULL	maximum photon energy	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : A Varian TrueBeam linac with a maximum photon energy of 15 MV was installed in asmaller , preexisting vault .
	manualset3
108296	4	402870	5	NULL	NULL	0	NULL	15 MV	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : A Varian TrueBeam linac with a maximum photon energy of 15 MV was installed in asmaller , preexisting vault .
	manualset3
108297	5	402870	5	NULL	NULL	0	NULL	smaller , preexisting vault	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : A Varian TrueBeam linac with a maximum photon energy of 15 MV was installed in asmaller , preexisting vault .
	manualset3
108298	1	402871	5	NULL	NULL	0	NULL	Methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : An algorithm is developed to program the existing XCAT phantom to move according to recorded patient 3D lung trajectory data .
	manualset3
108299	2	402871	5	NULL	NULL	0	NULL	algorithm	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : An algorithm is developed to program the existing XCAT phantom to move according to recorded patient 3D lung trajectory data .
	manualset3
108308	3	402871	5	NULL	NULL	NULL	NULL	XCAT phantom	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Methods : An algorithm is developed to program the existing XCAT phantom to move according to recorded patient 3D lung trajectory data .
	manualset3
108309	4	402871	5	NULL	NULL	NULL	NULL	patient	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Methods : An algorithm is developed to program the existing XCAT phantom to move according to recorded patient 3D lung trajectory data .
	manualset3
108310	5	402871	5	NULL	NULL	NULL	NULL	3D lung trajectory data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Methods : An algorithm is developed to program the existing XCAT phantom to move according to recorded patient 3D lung trajectory data .
	manualset3
108311	1	402872	5	NULL	NULL	0	NULL	Methods 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : Five patients ( 9 to 23 months of age ) with a diagnosis of long-segment aortic coarctation underwent conventional SFA .
	manualset3
108312	2	402872	5	NULL	NULL	0	NULL	Five patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : Five patients ( 9 to 23 months of age ) with a diagnosis of long-segment aortic coarctation underwent conventional SFA .
	manualset3
108313	3	402872	5	NULL	NULL	0	NULL	9 to 23 months of age	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : Five patients ( 9 to 23 months of age ) with a diagnosis of long-segment aortic coarctation underwent conventional SFA .
	manualset3
108314	4	402872	5	NULL	NULL	NULL	NULL	diagnosis 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Methods : Five patients ( 9 to 23 months of age ) with a diagnosis of long-segment aortic coarctation underwent conventional SFA .
	manualset3
108315	5	402872	5	NULL	NULL	0	NULL	long-segment aortic coarctation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : Five patients ( 9 to 23 months of age ) with a diagnosis of long-segment aortic coarctation underwent conventional SFA .
	manualset3
108316	6	402872	5	NULL	NULL	0	NULL	conventional SFA	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : Five patients ( 9 to 23 months of age ) with a diagnosis of long-segment aortic coarctation underwent conventional SFA .
	manualset3
108317	1	402873	5	NULL	NULL	0	NULL	Methods 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : Microscopic examination of stained thick and thin blood smears for the detection , quantification and specification of Plasmodium sp was performed on 493 blood donors in two main hospitals in Yaound during October and November 2007 .
	manualset3
108318	2	402873	5	NULL	NULL	0	NULL	Microscopic examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : Microscopic examination of stained thick and thin blood smears for the detection , quantification and specification of Plasmodium sp was performed on 493 blood donors in two main hospitals in Yaound during October and November 2007 .
	manualset3
108319	3	402873	5	NULL	NULL	0	NULL	stained thick blood smear	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : Microscopic examination of stained thick and thin blood smears for the detection , quantification and specification of Plasmodium sp was performed on 493 blood donors in two main hospitals in Yaound during October and November 2007 .
	manualset3
108320	4	402873	5	NULL	NULL	0	NULL	stained thin blood smear	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : Microscopic examination of stained thick and thin blood smears for the detection , quantification and specification of Plasmodium sp was performed on 493 blood donors in two main hospitals in Yaound during October and November 2007 .
	manualset3
108321	5	402873	5	NULL	NULL	0	NULL	detection 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : Microscopic examination of stained thick and thin blood smears for the detection , quantification and specification of Plasmodium sp was performed on 493 blood donors in two main hospitals in Yaound during October and November 2007 .
	manualset3
108322	6	402873	5	NULL	NULL	0	NULL	quantification 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : Microscopic examination of stained thick and thin blood smears for the detection , quantification and specification of Plasmodium sp was performed on 493 blood donors in two main hospitals in Yaound during October and November 2007 .
	manualset3
108323	7	402873	5	NULL	NULL	0	NULL	specification 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : Microscopic examination of stained thick and thin blood smears for the detection , quantification and specification of Plasmodium sp was performed on 493 blood donors in two main hospitals in Yaound during October and November 2007 .
	manualset3
108324	8	402873	5	NULL	NULL	0	NULL	Plasmodium sp 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : Microscopic examination of stained thick and thin blood smears for the detection , quantification and specification of Plasmodium sp was performed on 493 blood donors in two main hospitals in Yaound during October and November 2007 .
	manualset3
108325	9	402873	5	NULL	NULL	0	NULL	493 blood donors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : Microscopic examination of stained thick and thin blood smears for the detection , quantification and specification of Plasmodium sp was performed on 493 blood donors in two main hospitals in Yaound during October and November 2007 .
	manualset3
108326	10	402873	5	NULL	NULL	0	NULL	hospitals 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : Microscopic examination of stained thick and thin blood smears for the detection , quantification and specification of Plasmodium sp was performed on 493 blood donors in two main hospitals in Yaound during October and November 2007 .
	manualset3
108327	11	402873	5	NULL	NULL	0	NULL	Yaound 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : Microscopic examination of stained thick and thin blood smears for the detection , quantification and specification of Plasmodium sp was performed on 493 blood donors in two main hospitals in Yaound during October and November 2007 .
	manualset3
108328	12	402873	5	NULL	NULL	0	NULL	October 2007	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : Microscopic examination of stained thick and thin blood smears for the detection , quantification and specification of Plasmodium sp was performed on 493 blood donors in two main hospitals in Yaound during October and November 2007 .
	manualset3
108329	13	402873	5	NULL	NULL	0	NULL	November 2007	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : Microscopic examination of stained thick and thin blood smears for the detection , quantification and specification of Plasmodium sp was performed on 493 blood donors in two main hospitals in Yaound during October and November 2007 .
	manualset3
108330	1	402874	5	NULL	NULL	0	NULL	cDNA library	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A cDNA library from an HTLV-I-infected rabbit T-cell line was screened with p13K30 and p13K34 as bait .
	manualset3
108331	2	402874	5	NULL	NULL	0	NULL	HTLV-I-infected rabbit T-cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A cDNA library from an HTLV-I-infected rabbit T-cell line was screened with p13K30 and p13K34 as bait .
	manualset3
108332	3	402874	5	NULL	NULL	NULL	NULL	p13K30	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A cDNA library from an HTLV-I-infected rabbit T-cell line was screened with p13K30 and p13K34 as bait .
	manualset3
108333	4	402874	5	NULL	NULL	0	NULL	p13K34	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A cDNA library from an HTLV-I-infected rabbit T-cell line was screened with p13K30 and p13K34 as bait .
	manualset3
108334	5	402874	5	NULL	NULL	0	NULL	bait	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A cDNA library from an HTLV-I-infected rabbit T-cell line was screened with p13K30 and p13K34 as bait .
	manualset3
108335	1	402875	5	NULL	NULL	0	NULL	Methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : The glycemic responses elicited by portions of 4 individual foods with 25 g of available carbohydrate when served alone ( rice , lacy pancake , flatbread and noodles ) and when made into typical Malaysian mixed meals ( coconut milk rice , lacy pancake with chicken curry , flatbread with dhal curry and fried noodles ) were measured in 10 subjects with type 2 diabetes .
	manualset3
108336	2	402875	5	NULL	NULL	0	NULL	glycemic responses	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : The glycemic responses elicited by portions of 4 individual foods with 25 g of available carbohydrate when served alone ( rice , lacy pancake , flatbread and noodles ) and when made into typical Malaysian mixed meals ( coconut milk rice , lacy pancake with chicken curry , flatbread with dhal curry and fried noodles ) were measured in 10 subjects with type 2 diabetes .
	manualset3
108337	3	402875	5	NULL	NULL	0	NULL	portions 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : The glycemic responses elicited by portions of 4 individual foods with 25 g of available carbohydrate when served alone ( rice , lacy pancake , flatbread and noodles ) and when made into typical Malaysian mixed meals ( coconut milk rice , lacy pancake with chicken curry , flatbread with dhal curry and fried noodles ) were measured in 10 subjects with type 2 diabetes .
	manualset3
108338	4	402875	5	NULL	NULL	0	NULL	4 individual foods	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : The glycemic responses elicited by portions of 4 individual foods with 25 g of available carbohydrate when served alone ( rice , lacy pancake , flatbread and noodles ) and when made into typical Malaysian mixed meals ( coconut milk rice , lacy pancake with chicken curry , flatbread with dhal curry and fried noodles ) were measured in 10 subjects with type 2 diabetes .
	manualset3
108339	5	402875	5	NULL	NULL	0	NULL	25 g	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : The glycemic responses elicited by portions of 4 individual foods with 25 g of available carbohydrate when served alone ( rice , lacy pancake , flatbread and noodles ) and when made into typical Malaysian mixed meals ( coconut milk rice , lacy pancake with chicken curry , flatbread with dhal curry and fried noodles ) were measured in 10 subjects with type 2 diabetes .
	manualset3
108340	6	402875	5	NULL	NULL	0	NULL	available carbohydrate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : The glycemic responses elicited by portions of 4 individual foods with 25 g of available carbohydrate when served alone ( rice , lacy pancake , flatbread and noodles ) and when made into typical Malaysian mixed meals ( coconut milk rice , lacy pancake with chicken curry , flatbread with dhal curry and fried noodles ) were measured in 10 subjects with type 2 diabetes .
	manualset3
108341	7	402875	5	NULL	NULL	0	NULL	rice 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : The glycemic responses elicited by portions of 4 individual foods with 25 g of available carbohydrate when served alone ( rice , lacy pancake , flatbread and noodles ) and when made into typical Malaysian mixed meals ( coconut milk rice , lacy pancake with chicken curry , flatbread with dhal curry and fried noodles ) were measured in 10 subjects with type 2 diabetes .
	manualset3
108342	8	402875	5	NULL	NULL	0	NULL	lacy pancake	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : The glycemic responses elicited by portions of 4 individual foods with 25 g of available carbohydrate when served alone ( rice , lacy pancake , flatbread and noodles ) and when made into typical Malaysian mixed meals ( coconut milk rice , lacy pancake with chicken curry , flatbread with dhal curry and fried noodles ) were measured in 10 subjects with type 2 diabetes .
	manualset3
108343	9	402875	5	NULL	NULL	0	NULL	flatbread 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : The glycemic responses elicited by portions of 4 individual foods with 25 g of available carbohydrate when served alone ( rice , lacy pancake , flatbread and noodles ) and when made into typical Malaysian mixed meals ( coconut milk rice , lacy pancake with chicken curry , flatbread with dhal curry and fried noodles ) were measured in 10 subjects with type 2 diabetes .
	manualset3
108344	10	402875	5	NULL	NULL	0	NULL	noodles 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : The glycemic responses elicited by portions of 4 individual foods with 25 g of available carbohydrate when served alone ( rice , lacy pancake , flatbread and noodles ) and when made into typical Malaysian mixed meals ( coconut milk rice , lacy pancake with chicken curry , flatbread with dhal curry and fried noodles ) were measured in 10 subjects with type 2 diabetes .
	manualset3
108345	11	402875	5	NULL	NULL	0	NULL	Malaysian mixed meals	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : The glycemic responses elicited by portions of 4 individual foods with 25 g of available carbohydrate when served alone ( rice , lacy pancake , flatbread and noodles ) and when made into typical Malaysian mixed meals ( coconut milk rice , lacy pancake with chicken curry , flatbread with dhal curry and fried noodles ) were measured in 10 subjects with type 2 diabetes .
	manualset3
108346	12	402875	5	NULL	NULL	0	NULL	coconut milk rice	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : The glycemic responses elicited by portions of 4 individual foods with 25 g of available carbohydrate when served alone ( rice , lacy pancake , flatbread and noodles ) and when made into typical Malaysian mixed meals ( coconut milk rice , lacy pancake with chicken curry , flatbread with dhal curry and fried noodles ) were measured in 10 subjects with type 2 diabetes .
	manualset3
108347	13	402875	5	NULL	NULL	0	NULL	lacy pancake	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : The glycemic responses elicited by portions of 4 individual foods with 25 g of available carbohydrate when served alone ( rice , lacy pancake , flatbread and noodles ) and when made into typical Malaysian mixed meals ( coconut milk rice , lacy pancake with chicken curry , flatbread with dhal curry and fried noodles ) were measured in 10 subjects with type 2 diabetes .
	manualset3
108348	14	402875	5	NULL	NULL	0	NULL	chicken curry	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : The glycemic responses elicited by portions of 4 individual foods with 25 g of available carbohydrate when served alone ( rice , lacy pancake , flatbread and noodles ) and when made into typical Malaysian mixed meals ( coconut milk rice , lacy pancake with chicken curry , flatbread with dhal curry and fried noodles ) were measured in 10 subjects with type 2 diabetes .
	manualset3
108349	15	402875	5	NULL	NULL	0	NULL	flatbread 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : The glycemic responses elicited by portions of 4 individual foods with 25 g of available carbohydrate when served alone ( rice , lacy pancake , flatbread and noodles ) and when made into typical Malaysian mixed meals ( coconut milk rice , lacy pancake with chicken curry , flatbread with dhal curry and fried noodles ) were measured in 10 subjects with type 2 diabetes .
	manualset3
108350	16	402875	5	NULL	NULL	0	NULL	dhal curry	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : The glycemic responses elicited by portions of 4 individual foods with 25 g of available carbohydrate when served alone ( rice , lacy pancake , flatbread and noodles ) and when made into typical Malaysian mixed meals ( coconut milk rice , lacy pancake with chicken curry , flatbread with dhal curry and fried noodles ) were measured in 10 subjects with type 2 diabetes .
	manualset3
108351	17	402875	5	NULL	NULL	0	NULL	fried noodles 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : The glycemic responses elicited by portions of 4 individual foods with 25 g of available carbohydrate when served alone ( rice , lacy pancake , flatbread and noodles ) and when made into typical Malaysian mixed meals ( coconut milk rice , lacy pancake with chicken curry , flatbread with dhal curry and fried noodles ) were measured in 10 subjects with type 2 diabetes .
	manualset3
108352	18	402875	5	NULL	NULL	0	NULL	10 subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : The glycemic responses elicited by portions of 4 individual foods with 25 g of available carbohydrate when served alone ( rice , lacy pancake , flatbread and noodles ) and when made into typical Malaysian mixed meals ( coconut milk rice , lacy pancake with chicken curry , flatbread with dhal curry and fried noodles ) were measured in 10 subjects with type 2 diabetes .
	manualset3
108353	19	402875	5	NULL	NULL	0	NULL	type 2 diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : The glycemic responses elicited by portions of 4 individual foods with 25 g of available carbohydrate when served alone ( rice , lacy pancake , flatbread and noodles ) and when made into typical Malaysian mixed meals ( coconut milk rice , lacy pancake with chicken curry , flatbread with dhal curry and fried noodles ) were measured in 10 subjects with type 2 diabetes .
	manualset3
108354	1	402876	5	NULL	NULL	0	NULL	Methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : This is a sub-analysis of 564 patients of Mexico , extracted from an international , observational , and cross-sectional study followed by specialists , The study included patients with SAH without any other causes of microalbuminuria .
	manualset3
108355	2	402876	5	NULL	NULL	0	NULL	sub-analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : This is a sub-analysis of 564 patients of Mexico , extracted from an international , observational , and cross-sectional study followed by specialists , The study included patients with SAH without any other causes of microalbuminuria .
	manualset3
108356	3	402876	5	NULL	NULL	0	NULL	564 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : This is a sub-analysis of 564 patients of Mexico , extracted from an international , observational , and cross-sectional study followed by specialists , The study included patients with SAH without any other causes of microalbuminuria .
	manualset3
108357	4	402876	5	NULL	NULL	0	NULL	Mexico 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : This is a sub-analysis of 564 patients of Mexico , extracted from an international , observational , and cross-sectional study followed by specialists , The study included patients with SAH without any other causes of microalbuminuria .
	manualset3
108358	5	402876	5	NULL	NULL	0	NULL	international study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : This is a sub-analysis of 564 patients of Mexico , extracted from an international , observational , and cross-sectional study followed by specialists , The study included patients with SAH without any other causes of microalbuminuria .
	manualset3
108359	6	402876	5	NULL	NULL	0	NULL	observational study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : This is a sub-analysis of 564 patients of Mexico , extracted from an international , observational , and cross-sectional study followed by specialists , The study included patients with SAH without any other causes of microalbuminuria .
	manualset3
108360	7	402876	5	NULL	NULL	0	NULL	cross-sectional study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : This is a sub-analysis of 564 patients of Mexico , extracted from an international , observational , and cross-sectional study followed by specialists , The study included patients with SAH without any other causes of microalbuminuria .
	manualset3
108361	8	402876	5	NULL	NULL	0	NULL	specialists 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : This is a sub-analysis of 564 patients of Mexico , extracted from an international , observational , and cross-sectional study followed by specialists , The study included patients with SAH without any other causes of microalbuminuria .
	manualset3
108362	9	402876	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : This is a sub-analysis of 564 patients of Mexico , extracted from an international , observational , and cross-sectional study followed by specialists , The study included patients with SAH without any other causes of microalbuminuria .
	manualset3
108363	10	402876	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : This is a sub-analysis of 564 patients of Mexico , extracted from an international , observational , and cross-sectional study followed by specialists , The study included patients with SAH without any other causes of microalbuminuria .
	manualset3
108364	11	402876	5	NULL	NULL	0	NULL	SAH	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : This is a sub-analysis of 564 patients of Mexico , extracted from an international , observational , and cross-sectional study followed by specialists , The study included patients with SAH without any other causes of microalbuminuria .
	manualset3
108365	12	402876	5	NULL	NULL	0	NULL	microalbuminuria 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : This is a sub-analysis of 564 patients of Mexico , extracted from an international , observational , and cross-sectional study followed by specialists , The study included patients with SAH without any other causes of microalbuminuria .
	manualset3
108366	1	402877	5	NULL	NULL	0	NULL	Methods 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : We examined low birth weight ( LBW ) , preterm birth , fetal growth restriction , and birth defects among births to women in Endicott who were exposed to VOCs , compared with births statewide .
	manualset3
108367	2	402877	5	NULL	NULL	0	NULL	low birth weight ( LBW )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : We examined low birth weight ( LBW ) , preterm birth , fetal growth restriction , and birth defects among births to women in Endicott who were exposed to VOCs , compared with births statewide .
	manualset3
108368	3	402877	5	NULL	NULL	0	NULL	preterm birth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : We examined low birth weight ( LBW ) , preterm birth , fetal growth restriction , and birth defects among births to women in Endicott who were exposed to VOCs , compared with births statewide .
	manualset3
108369	4	402877	5	NULL	NULL	0	NULL	fetal growth restriction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : We examined low birth weight ( LBW ) , preterm birth , fetal growth restriction , and birth defects among births to women in Endicott who were exposed to VOCs , compared with births statewide .
	manualset3
108370	5	402877	5	NULL	NULL	0	NULL	birth defects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : We examined low birth weight ( LBW ) , preterm birth , fetal growth restriction , and birth defects among births to women in Endicott who were exposed to VOCs , compared with births statewide .
	manualset3
108371	6	402877	5	NULL	NULL	0	NULL	births 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : We examined low birth weight ( LBW ) , preterm birth , fetal growth restriction , and birth defects among births to women in Endicott who were exposed to VOCs , compared with births statewide .
	manualset3
108372	7	402877	5	NULL	NULL	0	NULL	women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : We examined low birth weight ( LBW ) , preterm birth , fetal growth restriction , and birth defects among births to women in Endicott who were exposed to VOCs , compared with births statewide .
	manualset3
108373	8	402877	5	NULL	NULL	0	NULL	Endicott 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : We examined low birth weight ( LBW ) , preterm birth , fetal growth restriction , and birth defects among births to women in Endicott who were exposed to VOCs , compared with births statewide .
	manualset3
108374	9	402877	5	NULL	NULL	0	NULL	VOCs 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : We examined low birth weight ( LBW ) , preterm birth , fetal growth restriction , and birth defects among births to women in Endicott who were exposed to VOCs , compared with births statewide .
	manualset3
108375	10	402877	5	NULL	NULL	0	NULL	births 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : We examined low birth weight ( LBW ) , preterm birth , fetal growth restriction , and birth defects among births to women in Endicott who were exposed to VOCs , compared with births statewide .
	manualset3
108376	1	402878	5	NULL	NULL	0	NULL	Methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : We used TOPAS , a new MC simulation tool that provides a user-friendly interface to the Geant4 package , to simulate proton depth-dose curves from the MGH gantry treatment heads in double - scattering mode .
	manualset3
108377	2	402878	5	NULL	NULL	0	NULL	TOPAS 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : We used TOPAS , a new MC simulation tool that provides a user-friendly interface to the Geant4 package , to simulate proton depth-dose curves from the MGH gantry treatment heads in double - scattering mode .
	manualset3
108378	3	402878	5	NULL	NULL	0	NULL	MC simulation tool	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : We used TOPAS , a new MC simulation tool that provides a user-friendly interface to the Geant4 package , to simulate proton depth-dose curves from the MGH gantry treatment heads in double - scattering mode .
	manualset3
108379	4	402878	5	NULL	NULL	0	NULL	user-friendly interface	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : We used TOPAS , a new MC simulation tool that provides a user-friendly interface to the Geant4 package , to simulate proton depth-dose curves from the MGH gantry treatment heads in double - scattering mode .
	manualset3
108380	5	402878	5	NULL	NULL	0	NULL	Geant4 package	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : We used TOPAS , a new MC simulation tool that provides a user-friendly interface to the Geant4 package , to simulate proton depth-dose curves from the MGH gantry treatment heads in double - scattering mode .
	manualset3
108381	6	402878	5	NULL	NULL	0	NULL	proton depth-dose curves	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : We used TOPAS , a new MC simulation tool that provides a user-friendly interface to the Geant4 package , to simulate proton depth-dose curves from the MGH gantry treatment heads in double - scattering mode .
	manualset3
108382	7	402878	5	NULL	NULL	0	NULL	MGH gantry treatment heads	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : We used TOPAS , a new MC simulation tool that provides a user-friendly interface to the Geant4 package , to simulate proton depth-dose curves from the MGH gantry treatment heads in double - scattering mode .
	manualset3
108383	8	402878	5	NULL	NULL	NULL	NULL	double - scattering mode	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Methods : We used TOPAS , a new MC simulation tool that provides a user-friendly interface to the Geant4 package , to simulate proton depth-dose curves from the MGH gantry treatment heads in double - scattering mode .
	manualset3
108384	1	402879	5	NULL	NULL	0	NULL	Methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods Antiaquaporin-4 antibody ( AQP4-ab ) levels were tested in 2366 serum samples of patients diagnosed as having central nervous system inflammatory demyelinating disorders by their referring physicians .
	manualset3
108385	2	402879	5	NULL	NULL	0	NULL	Antiaquaporin-4 antibody ( AQP4-ab ) levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods Antiaquaporin-4 antibody ( AQP4-ab ) levels were tested in 2366 serum samples of patients diagnosed as having central nervous system inflammatory demyelinating disorders by their referring physicians .
	manualset3
108387	4	402879	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods Antiaquaporin-4 antibody ( AQP4-ab ) levels were tested in 2366 serum samples of patients diagnosed as having central nervous system inflammatory demyelinating disorders by their referring physicians .
	manualset3
108388	5	402879	5	NULL	NULL	0	NULL	central nervous system inflammatory demyelinating disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods Antiaquaporin-4 antibody ( AQP4-ab ) levels were tested in 2366 serum samples of patients diagnosed as having central nervous system inflammatory demyelinating disorders by their referring physicians .
	manualset3
108389	6	402879	5	NULL	NULL	0	NULL	referring physicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods Antiaquaporin-4 antibody ( AQP4-ab ) levels were tested in 2366 serum samples of patients diagnosed as having central nervous system inflammatory demyelinating disorders by their referring physicians .
	manualset3
113859	3	402879	5	NULL	NULL	0	NULL	2366 serum samples	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods Antiaquaporin-4 antibody ( AQP4-ab ) levels were tested in 2366 serum samples of patients diagnosed as having central nervous system inflammatory demyelinating disorders by their referring physicians .
	manualset3
108391	1	402880	5	NULL	NULL	0	NULL	Methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods This study included 17 children who were diagnosed with Peutz-Jeghers syndrome based on clinical diagnostic criteria between July 2006 and December 2007 .
	manualset3
108392	2	402880	5	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods This study included 17 children who were diagnosed with Peutz-Jeghers syndrome based on clinical diagnostic criteria between July 2006 and December 2007 .
	manualset3
108393	3	402880	5	NULL	NULL	0	NULL	17 children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods This study included 17 children who were diagnosed with Peutz-Jeghers syndrome based on clinical diagnostic criteria between July 2006 and December 2007 .
	manualset3
108394	4	402880	5	NULL	NULL	NULL	NULL	Peutz-Jeghers syndrome	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Methods This study included 17 children who were diagnosed with Peutz-Jeghers syndrome based on clinical diagnostic criteria between July 2006 and December 2007 .
	manualset3
108395	5	402880	5	NULL	NULL	0	NULL	clinical diagnostic criteria	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods This study included 17 children who were diagnosed with Peutz-Jeghers syndrome based on clinical diagnostic criteria between July 2006 and December 2007 .
	manualset3
108396	6	402880	5	NULL	NULL	0	NULL	July 2006	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods This study included 17 children who were diagnosed with Peutz-Jeghers syndrome based on clinical diagnostic criteria between July 2006 and December 2007 .
	manualset3
108397	7	402880	5	NULL	NULL	0	NULL	December 2007	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods This study included 17 children who were diagnosed with Peutz-Jeghers syndrome based on clinical diagnostic criteria between July 2006 and December 2007 .
	manualset3
108398	1	402881	5	NULL	NULL	0	NULL	Methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods and results One hundred and eighty-six asymptomatic patients with at least moderate AS and preserved LV ejection fraction ( ) / = 50 % ) were assessed by Doppler-echocardiography at rest and during a maximum ramp semi-supine bicycle exercise test .
	manualset3
108399	2	402881	5	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods and results One hundred and eighty-six asymptomatic patients with at least moderate AS and preserved LV ejection fraction ( ) / = 50 % ) were assessed by Doppler-echocardiography at rest and during a maximum ramp semi-supine bicycle exercise test .
	manualset3
108400	3	402881	5	NULL	NULL	0	NULL	One hundred and eighty-six asymptomatic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods and results One hundred and eighty-six asymptomatic patients with at least moderate AS and preserved LV ejection fraction ( ) / = 50 % ) were assessed by Doppler-echocardiography at rest and during a maximum ramp semi-supine bicycle exercise test .
	manualset3
108401	4	402881	5	NULL	NULL	0	NULL	least moderate AS ejection fraction 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods and results One hundred and eighty-six asymptomatic patients with at least moderate AS and preserved LV ejection fraction ( ) / = 50 % ) were assessed by Doppler-echocardiography at rest and during a maximum ramp semi-supine bicycle exercise test .
	manualset3
108402	5	402881	5	NULL	NULL	0	NULL	preserved LV ejection fraction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods and results One hundred and eighty-six asymptomatic patients with at least moderate AS and preserved LV ejection fraction ( ) / = 50 % ) were assessed by Doppler-echocardiography at rest and during a maximum ramp semi-supine bicycle exercise test .
	manualset3
108403	6	402881	5	NULL	NULL	0	NULL	/ = 50 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods and results One hundred and eighty-six asymptomatic patients with at least moderate AS and preserved LV ejection fraction ( ) / = 50 % ) were assessed by Doppler-echocardiography at rest and during a maximum ramp semi-supine bicycle exercise test .
	manualset3
108404	7	402881	5	NULL	NULL	0	NULL	Doppler-echocardiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods and results One hundred and eighty-six asymptomatic patients with at least moderate AS and preserved LV ejection fraction ( ) / = 50 % ) were assessed by Doppler-echocardiography at rest and during a maximum ramp semi-supine bicycle exercise test .
	manualset3
108405	8	402881	5	NULL	NULL	0	NULL	maximum ramp semi-supine bicycle exercise test	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods and results One hundred and eighty-six asymptomatic patients with at least moderate AS and preserved LV ejection fraction ( ) / = 50 % ) were assessed by Doppler-echocardiography at rest and during a maximum ramp semi-supine bicycle exercise test .
	manualset3
108406	1	402882	5	NULL	NULL	0	NULL	Methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods are proposed for reducing the number of sensors required and increasing the lifetime of those used , for considerably reduced energy consumption .
	manualset3
108407	2	402882	5	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods are proposed for reducing the number of sensors required and increasing the lifetime of those used , for considerably reduced energy consumption .
	manualset3
108408	3	402882	5	NULL	NULL	0	NULL	sensors 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods are proposed for reducing the number of sensors required and increasing the lifetime of those used , for considerably reduced energy consumption .
	manualset3
108409	4	402882	5	NULL	NULL	0	NULL	lifetime 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods are proposed for reducing the number of sensors required and increasing the lifetime of those used , for considerably reduced energy consumption .
	manualset3
108410	5	402882	5	NULL	NULL	0	NULL	reduced energy consumption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods are proposed for reducing the number of sensors required and increasing the lifetime of those used , for considerably reduced energy consumption .
	manualset3
108411	1	402883	5	NULL	NULL	0	NULL	capsid	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A capsid originating from prion proteins would be a versatile and effective protection to RNA and could also explain some characteristics of virus self-assembly that are not well understood .
	manualset3
108412	2	402883	5	NULL	NULL	0	NULL	prion proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A capsid originating from prion proteins would be a versatile and effective protection to RNA and could also explain some characteristics of virus self-assembly that are not well understood .
	manualset3
108413	3	402883	5	NULL	NULL	0	NULL	RNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A capsid originating from prion proteins would be a versatile and effective protection to RNA and could also explain some characteristics of virus self-assembly that are not well understood .
	manualset3
108414	4	402883	5	NULL	NULL	0	NULL	virus self-assembly 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A capsid originating from prion proteins would be a versatile and effective protection to RNA and could also explain some characteristics of virus self-assembly that are not well understood .
	manualset3
108415	1	402884	5	NULL	NULL	0	NULL	Methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods to reduce background interferences in electron-capture gas chromatographic analysis of valproic acid and its unsaturated metabolites after derivatization with pentafluorobenzyl bromide .
	manualset3
108416	2	402884	5	NULL	NULL	0	NULL	background interferences	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods to reduce background interferences in electron-capture gas chromatographic analysis of valproic acid and its unsaturated metabolites after derivatization with pentafluorobenzyl bromide .
	manualset3
108417	3	402884	5	NULL	NULL	0	NULL	electron-capture gas chromatographic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods to reduce background interferences in electron-capture gas chromatographic analysis of valproic acid and its unsaturated metabolites after derivatization with pentafluorobenzyl bromide .
	manualset3
108418	4	402884	5	NULL	NULL	0	NULL	valproic acid	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods to reduce background interferences in electron-capture gas chromatographic analysis of valproic acid and its unsaturated metabolites after derivatization with pentafluorobenzyl bromide .
	manualset3
108419	5	402884	5	NULL	NULL	0	NULL	unsaturated metabolites 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods to reduce background interferences in electron-capture gas chromatographic analysis of valproic acid and its unsaturated metabolites after derivatization with pentafluorobenzyl bromide .
	manualset3
108420	6	402884	5	NULL	NULL	0	NULL	derivatization 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods to reduce background interferences in electron-capture gas chromatographic analysis of valproic acid and its unsaturated metabolites after derivatization with pentafluorobenzyl bromide .
	manualset3
108421	7	402884	5	NULL	NULL	0	NULL	pentafluorobenzyl bromide	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods to reduce background interferences in electron-capture gas chromatographic analysis of valproic acid and its unsaturated metabolites after derivatization with pentafluorobenzyl bromide .
	manualset3
108422	1	402885	5	NULL	NULL	0	NULL	Methotrexate AUC	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Methotrexate AUC was significantly higher in girls than boys ( P = .007 ) .
	manualset3
108423	2	402885	5	NULL	NULL	0	NULL	girls 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Methotrexate AUC was significantly higher in girls than boys ( P = .007 ) .
	manualset3
108424	3	402885	5	NULL	NULL	0	NULL	boys 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Methotrexate AUC was significantly higher in girls than boys ( P = .007 ) .
	manualset3
108425	4	402885	5	NULL	NULL	0	NULL	P = .007	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Methotrexate AUC was significantly higher in girls than boys ( P = .007 ) .
	manualset3
108426	1	402886	5	NULL	NULL	0	NULL	Methotrexate delivery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Methotrexate delivery to the eye using transscleral hydrogel iontophoresis .
	manualset3
108427	2	402886	5	NULL	NULL	0	NULL	eye 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Methotrexate delivery to the eye using transscleral hydrogel iontophoresis .
	manualset3
108428	3	402886	5	NULL	NULL	0	NULL	transscleral hydrogel iontophoresis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Methotrexate delivery to the eye using transscleral hydrogel iontophoresis .
	manualset3
108429	1	402887	5	NULL	NULL	0	NULL	Methyl-beta-D-thiogalactoside	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Methyl-beta-D-thiogalactoside , a substrate for both systems , inhibited the transport of melibiose via both systems .
	manualset3
108430	2	402887	5	NULL	NULL	0	NULL	substrate 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Methyl-beta-D-thiogalactoside , a substrate for both systems , inhibited the transport of melibiose via both systems .
	manualset3
108431	3	402887	5	NULL	NULL	0	NULL	both systems	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methyl-beta-D-thiogalactoside , a substrate for both systems , inhibited the transport of melibiose via both systems .
	manualset3
108432	4	402887	5	NULL	NULL	0	NULL	melibiose 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Methyl-beta-D-thiogalactoside , a substrate for both systems , inhibited the transport of melibiose via both systems .
	manualset3
108433	5	402887	5	NULL	NULL	0	NULL	both systems 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methyl-beta-D-thiogalactoside , a substrate for both systems , inhibited the transport of melibiose via both systems .
	manualset3
108434	1	402888	5	NULL	NULL	0	NULL	Methyl-coenzyme-M reductase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Methyl-coenzyme-M reductase from Methanobacterium thermoautotrophicum ( strain Marburg ) .
	manualset3
108435	2	402888	5	NULL	NULL	0	NULL	Methanobacterium thermoautotrophicum ( strain Marburg )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Methyl-coenzyme-M reductase from Methanobacterium thermoautotrophicum ( strain Marburg ) .
	manualset3
108436	1	402889	5	NULL	NULL	NULL	NULL	Methyl 4 , 6-O-benzylidene-2-deoxy-alpha-D-ribo-hexopyranoside 	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Methyl 4 , 6-O-benzylidene-2-deoxy-alpha-D-ribo-hexopyranoside ( 1 ) is converted into methyl 3 , 4-di-O-benzoyl-6-bromo-2 , 6 - dideoxy-alpha-D-ribo-hexopyranoside ( 3 ) via the 3-O-benzoyl derivative ( 2 ) of 1 by subsequent treatment with N-bromosuccinimide .
	manualset3
108437	2	402889	5	NULL	NULL	0	NULL	methyl 3,4-di-O-benzoyl-6-bromo-2,6-dideoxy-alpha-D-ribo-hexopyranoside	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Methyl 4 , 6-O-benzylidene-2-deoxy-alpha-D-ribo-hexopyranoside ( 1 ) is converted into methyl 3 , 4-di-O-benzoyl-6-bromo-2 , 6 - dideoxy-alpha-D-ribo-hexopyranoside ( 3 ) via the 3-O-benzoyl derivative ( 2 ) of 1 by subsequent treatment with N-bromosuccinimide .
	manualset3
108438	3	402889	5	NULL	NULL	0	NULL	3-O-benzoyl derivative of Methyl 4 , 6-O-benzylidene-2-deoxy-alpha-D-ribo-hexopyranoside 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Methyl 4 , 6-O-benzylidene-2-deoxy-alpha-D-ribo-hexopyranoside ( 1 ) is converted into methyl 3 , 4-di-O-benzoyl-6-bromo-2 , 6 - dideoxy-alpha-D-ribo-hexopyranoside ( 3 ) via the 3-O-benzoyl derivative ( 2 ) of 1 by subsequent treatment with N-bromosuccinimide .
	manualset3
108439	4	402889	5	NULL	NULL	0	NULL	treatment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methyl 4 , 6-O-benzylidene-2-deoxy-alpha-D-ribo-hexopyranoside ( 1 ) is converted into methyl 3 , 4-di-O-benzoyl-6-bromo-2 , 6 - dideoxy-alpha-D-ribo-hexopyranoside ( 3 ) via the 3-O-benzoyl derivative ( 2 ) of 1 by subsequent treatment with N-bromosuccinimide .
	manualset3
108440	5	402889	5	NULL	NULL	0	NULL	 N-bromosuccinimide 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Methyl 4 , 6-O-benzylidene-2-deoxy-alpha-D-ribo-hexopyranoside ( 1 ) is converted into methyl 3 , 4-di-O-benzoyl-6-bromo-2 , 6 - dideoxy-alpha-D-ribo-hexopyranoside ( 3 ) via the 3-O-benzoyl derivative ( 2 ) of 1 by subsequent treatment with N-bromosuccinimide .
	manualset3
108441	1	402890	5	NULL	NULL	0	NULL	Methyl mercury pretreatment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methyl mercury pretreatment per se of strain R rats on the standard diet gave no effect .
	manualset3
108442	2	402890	5	NULL	NULL	0	NULL	strain R rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Methyl mercury pretreatment per se of strain R rats on the standard diet gave no effect .
	manualset3
108443	3	402890	5	NULL	NULL	0	NULL	standard diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Methyl mercury pretreatment per se of strain R rats on the standard diet gave no effect .
	manualset3
108444	1	402891	5	NULL	NULL	0	NULL	Methylated proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Methylated proteins in 50 S ribosomes of E. coli EA2 .
	manualset3
108445	2	402891	5	NULL	NULL	0	NULL	50 S ribosomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Methylated proteins in 50 S ribosomes of E. coli EA2 .
	manualset3
108446	3	402891	5	NULL	NULL	0	NULL	E. coli EA2	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Methylated proteins in 50 S ribosomes of E. coli EA2 .
	manualset3
108447	1	402892	5	NULL	NULL	0	NULL	Methylation analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methylation analysis of the neurofibromatosis type 1 ( NF1 ) promoter in peripheral nerve sheath tumors .
	manualset3
108448	2	402892	5	NULL	NULL	0	NULL	neurofibromatosis type 1 ( NF1 ) promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Methylation analysis of the neurofibromatosis type 1 ( NF1 ) promoter in peripheral nerve sheath tumors .
	manualset3
108449	3	402892	5	NULL	NULL	0	NULL	peripheral nerve sheath tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Methylation analysis of the neurofibromatosis type 1 ( NF1 ) promoter in peripheral nerve sheath tumors .
	manualset3
108450	1	402893	5	NULL	NULL	NULL	NULL	Methylation 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Methylation could , therefore , play an important role in the increased risk of gynaecological malignancies in BRCA mutation carriers .
	manualset3
108451	2	402893	5	NULL	NULL	0	NULL	important role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Methylation could , therefore , play an important role in the increased risk of gynaecological malignancies in BRCA mutation carriers .
	manualset3
108452	3	402893	5	NULL	NULL	0	NULL	increased risk 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Methylation could , therefore , play an important role in the increased risk of gynaecological malignancies in BRCA mutation carriers .
	manualset3
108453	4	402893	5	NULL	NULL	0	NULL	gynaecological malignancies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Methylation could , therefore , play an important role in the increased risk of gynaecological malignancies in BRCA mutation carriers .
	manualset3
108454	5	402893	5	NULL	NULL	0	NULL	BRCA mutation carriers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Methylation could , therefore , play an important role in the increased risk of gynaecological malignancies in BRCA mutation carriers .
	manualset3
108455	1	402894	5	NULL	NULL	0	NULL	Methylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Methylation of CpG dinucleotides in the promoter region of the gene encoding the S100b protein in BALB/cLac mice .
	manualset3
108456	2	402894	5	NULL	NULL	0	NULL	CpG dinucleotides	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Methylation of CpG dinucleotides in the promoter region of the gene encoding the S100b protein in BALB/cLac mice .
	manualset3
108457	3	402894	5	NULL	NULL	0	NULL	promoter region 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Methylation of CpG dinucleotides in the promoter region of the gene encoding the S100b protein in BALB/cLac mice .
	manualset3
108458	4	402894	5	NULL	NULL	NULL	NULL	gene encoding the S100b protein	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Methylation of CpG dinucleotides in the promoter region of the gene encoding the S100b protein in BALB/cLac mice .
	manualset3
108459	5	402894	5	NULL	NULL	0	NULL	BALB/cLac mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Methylation of CpG dinucleotides in the promoter region of the gene encoding the S100b protein in BALB/cLac mice .
	manualset3
108460	1	402895	5	NULL	NULL	0	NULL	 care plan	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A care plan should be used as a link between the outpatient 's nurse and ward nurses involved with the patient 's primary care and the personnel in theater responsible for the patient .
	manualset3
108461	2	402895	5	NULL	NULL	0	NULL	link	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A care plan should be used as a link between the outpatient 's nurse and ward nurses involved with the patient 's primary care and the personnel in theater responsible for the patient .
	manualset3
108462	3	402895	5	NULL	NULL	0	NULL	outpatient 's nurse	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A care plan should be used as a link between the outpatient 's nurse and ward nurses involved with the patient 's primary care and the personnel in theater responsible for the patient .
	manualset3
108463	4	402895	5	NULL	NULL	0	NULL	ward nurses 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A care plan should be used as a link between the outpatient 's nurse and ward nurses involved with the patient 's primary care and the personnel in theater responsible for the patient .
	manualset3
108464	5	402895	5	NULL	NULL	0	NULL	patient 's primary care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A care plan should be used as a link between the outpatient 's nurse and ward nurses involved with the patient 's primary care and the personnel in theater responsible for the patient .
	manualset3
108465	6	402895	5	NULL	NULL	0	NULL	personnel 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A care plan should be used as a link between the outpatient 's nurse and ward nurses involved with the patient 's primary care and the personnel in theater responsible for the patient .
	manualset3
108466	7	402895	5	NULL	NULL	0	NULL	theater 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A care plan should be used as a link between the outpatient 's nurse and ward nurses involved with the patient 's primary care and the personnel in theater responsible for the patient .
	manualset3
108467	8	402895	5	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A care plan should be used as a link between the outpatient 's nurse and ward nurses involved with the patient 's primary care and the personnel in theater responsible for the patient .
	manualset3
108468	1	402896	5	NULL	NULL	NULL	NULL	Methylenedioxyphenyl insecticide synergists 	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Methylenedioxyphenyl insecticide synergists as potential human health hazards .
	manualset3
108469	2	402896	5	NULL	NULL	NULL	NULL	potential human health hazards	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Methylenedioxyphenyl insecticide synergists as potential human health hazards .
	manualset3
108470	1	402897	5	NULL	NULL	0	NULL	Methylenetetrahydrofolate reductase ( MTHFR ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Methylenetetrahydrofolate reductase ( MTHFR ) plays a central role in folate metabolism that affects DNA methylation and synthesis .
	manualset3
108471	2	402897	5	NULL	NULL	0	NULL	central role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Methylenetetrahydrofolate reductase ( MTHFR ) plays a central role in folate metabolism that affects DNA methylation and synthesis .
	manualset3
108472	3	402897	5	NULL	NULL	0	NULL	folate metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Methylenetetrahydrofolate reductase ( MTHFR ) plays a central role in folate metabolism that affects DNA methylation and synthesis .
	manualset3
108473	4	402897	5	NULL	NULL	0	NULL	DNA methylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Methylenetetrahydrofolate reductase ( MTHFR ) plays a central role in folate metabolism that affects DNA methylation and synthesis .
	manualset3
108474	5	402897	5	NULL	NULL	0	NULL	DNA synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Methylenetetrahydrofolate reductase ( MTHFR ) plays a central role in folate metabolism that affects DNA methylation and synthesis .
	manualset3
108475	1	402898	5	NULL	NULL	0	NULL	Methylmercury exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Methylmercury exposure in Northern Quebec II : neurologic findings in children .
	manualset3
108476	2	402898	5	NULL	NULL	0	NULL	Northern Quebec II	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Methylmercury exposure in Northern Quebec II : neurologic findings in children .
	manualset3
108477	3	402898	5	NULL	NULL	0	NULL	neurologic findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Methylmercury exposure in Northern Quebec II : neurologic findings in children .
	manualset3
108478	4	402898	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Methylmercury exposure in Northern Quebec II : neurologic findings in children .
	manualset3
108479	1	402899	5	NULL	NULL	0	NULL	Methylphenidate treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Methylphenidate treatment did not significantly affect height , weight , or overweight status .
	manualset3
108480	2	402899	5	NULL	NULL	0	NULL	height 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methylphenidate treatment did not significantly affect height , weight , or overweight status .
	manualset3
108481	3	402899	5	NULL	NULL	0	NULL	weight 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methylphenidate treatment did not significantly affect height , weight , or overweight status .
	manualset3
108482	4	402899	5	NULL	NULL	0	NULL	overweight status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Methylphenidate treatment did not significantly affect height , weight , or overweight status .
	manualset3
108483	1	402900	5	NULL	NULL	0	NULL	Metyrapone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Metyrapone or alpha-naphthoflavone inhibition of BP or 3-MC , respectively , markedly affected the production of free and conjugated metabolites and , almost completely , the deacetylation of 2-AAF .
	manualset3
108484	2	402900	5	NULL	NULL	0	NULL	inhibition 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Metyrapone or alpha-naphthoflavone inhibition of BP or 3-MC , respectively , markedly affected the production of free and conjugated metabolites and , almost completely , the deacetylation of 2-AAF .
	manualset3
108485	3	402900	5	NULL	NULL	0	NULL	BP 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Metyrapone or alpha-naphthoflavone inhibition of BP or 3-MC , respectively , markedly affected the production of free and conjugated metabolites and , almost completely , the deacetylation of 2-AAF .
	manualset3
108486	4	402900	5	NULL	NULL	0	NULL	3-MC 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Metyrapone or alpha-naphthoflavone inhibition of BP or 3-MC , respectively , markedly affected the production of free and conjugated metabolites and , almost completely , the deacetylation of 2-AAF .
	manualset3
108487	5	402900	5	NULL	NULL	0	NULL	production 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Metyrapone or alpha-naphthoflavone inhibition of BP or 3-MC , respectively , markedly affected the production of free and conjugated metabolites and , almost completely , the deacetylation of 2-AAF .
	manualset3
108488	6	402900	5	NULL	NULL	0	NULL	 free metabolites	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Metyrapone or alpha-naphthoflavone inhibition of BP or 3-MC , respectively , markedly affected the production of free and conjugated metabolites and , almost completely , the deacetylation of 2-AAF .
	manualset3
108489	7	402900	5	NULL	NULL	0	NULL	conjugated metabolites 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Metyrapone or alpha-naphthoflavone inhibition of BP or 3-MC , respectively , markedly affected the production of free and conjugated metabolites and , almost completely , the deacetylation of 2-AAF .
	manualset3
108490	8	402900	5	NULL	NULL	0	NULL	deacetylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Metyrapone or alpha-naphthoflavone inhibition of BP or 3-MC , respectively , markedly affected the production of free and conjugated metabolites and , almost completely , the deacetylation of 2-AAF .
	manualset3
108491	9	402900	5	NULL	NULL	0	NULL	2-AAF	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Metyrapone or alpha-naphthoflavone inhibition of BP or 3-MC , respectively , markedly affected the production of free and conjugated metabolites and , almost completely , the deacetylation of 2-AAF .
	manualset3
108492	1	402901	5	NULL	NULL	0	NULL	MeuTx3B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	MeuTx3B is an orthologue of BmTx3B/Martentoxin ( - KTx16 subfamily ) from Mesobuthus martensii that differs by three amino acid substitutions .
	manualset3
108493	2	402901	5	NULL	NULL	0	NULL	orthologue 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	MeuTx3B is an orthologue of BmTx3B/Martentoxin ( - KTx16 subfamily ) from Mesobuthus martensii that differs by three amino acid substitutions .
	manualset3
108494	3	402901	5	NULL	NULL	0	NULL	 BmTx3B/Martentoxin	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MeuTx3B is an orthologue of BmTx3B/Martentoxin ( - KTx16 subfamily ) from Mesobuthus martensii that differs by three amino acid substitutions .
	manualset3
108495	4	402901	5	NULL	NULL	0	NULL	 - KTx16 subfamily	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	MeuTx3B is an orthologue of BmTx3B/Martentoxin ( - KTx16 subfamily ) from Mesobuthus martensii that differs by three amino acid substitutions .
	manualset3
108496	5	402901	5	NULL	NULL	0	NULL	Mesobuthus martensii	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	MeuTx3B is an orthologue of BmTx3B/Martentoxin ( - KTx16 subfamily ) from Mesobuthus martensii that differs by three amino acid substitutions .
	manualset3
108497	6	402901	5	NULL	NULL	0	NULL	three amino acid substitutions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MeuTx3B is an orthologue of BmTx3B/Martentoxin ( - KTx16 subfamily ) from Mesobuthus martensii that differs by three amino acid substitutions .
	manualset3
108498	1	402902	5	NULL	NULL	0	NULL	Mg deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mg deficiency results in a stress effect and increased susceptibility to physiological damage produced by stress .
	manualset3
108499	2	402902	5	NULL	NULL	0	NULL	results 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mg deficiency results in a stress effect and increased susceptibility to physiological damage produced by stress .
	manualset3
108500	3	402902	5	NULL	NULL	0	NULL	stress effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mg deficiency results in a stress effect and increased susceptibility to physiological damage produced by stress .
	manualset3
108501	4	402902	5	NULL	NULL	0	NULL	susceptibility to physiological damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mg deficiency results in a stress effect and increased susceptibility to physiological damage produced by stress .
	manualset3
108502	5	402902	5	NULL	NULL	0	NULL	stress 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mg deficiency results in a stress effect and increased susceptibility to physiological damage produced by stress .
	manualset3
108503	1	402903	5	NULL	NULL	0	NULL	Mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice devoid of PrP are resistant to scrapie .
	manualset3
108504	2	402903	5	NULL	NULL	0	NULL	PrP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice devoid of PrP are resistant to scrapie .
	manualset3
108505	3	402903	5	NULL	NULL	0	NULL	scrapie 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice devoid of PrP are resistant to scrapie .
	manualset3
108506	1	402904	5	NULL	NULL	0	NULL	Mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice fed with a 2.0 % GF-containing diet ( GF2 .0 ) transiently exhibited phase advance or phase advance-like phenomenon by 1-3 h in terms of the biological rhythms of T ( b ) or LA , respectively ( both , P & lt ; 0.05 ) while mice were kept under conditions of a light/dark cycle ( 12 h : 12 h ) .
	manualset3
108507	2	402904	5	NULL	NULL	0	NULL	2.0 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice fed with a 2.0 % GF-containing diet ( GF2 .0 ) transiently exhibited phase advance or phase advance-like phenomenon by 1-3 h in terms of the biological rhythms of T ( b ) or LA , respectively ( both , P & lt ; 0.05 ) while mice were kept under conditions of a light/dark cycle ( 12 h : 12 h ) .
	manualset3
108508	3	402904	5	NULL	NULL	0	NULL	GF-containing diet ( GF2 .0 )	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice fed with a 2.0 % GF-containing diet ( GF2 .0 ) transiently exhibited phase advance or phase advance-like phenomenon by 1-3 h in terms of the biological rhythms of T ( b ) or LA , respectively ( both , P & lt ; 0.05 ) while mice were kept under conditions of a light/dark cycle ( 12 h : 12 h ) .
	manualset3
108509	4	402904	5	NULL	NULL	NULL	NULL	phase advance phenomenon 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mice fed with a 2.0 % GF-containing diet ( GF2 .0 ) transiently exhibited phase advance or phase advance-like phenomenon by 1-3 h in terms of the biological rhythms of T ( b ) or LA , respectively ( both , P & lt ; 0.05 ) while mice were kept under conditions of a light/dark cycle ( 12 h : 12 h ) .
	manualset3
108510	5	402904	5	NULL	NULL	0	NULL	phase advance-like phenomenon	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice fed with a 2.0 % GF-containing diet ( GF2 .0 ) transiently exhibited phase advance or phase advance-like phenomenon by 1-3 h in terms of the biological rhythms of T ( b ) or LA , respectively ( both , P & lt ; 0.05 ) while mice were kept under conditions of a light/dark cycle ( 12 h : 12 h ) .
	manualset3
108511	6	402904	5	NULL	NULL	0	NULL	1-3 h 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice fed with a 2.0 % GF-containing diet ( GF2 .0 ) transiently exhibited phase advance or phase advance-like phenomenon by 1-3 h in terms of the biological rhythms of T ( b ) or LA , respectively ( both , P & lt ; 0.05 ) while mice were kept under conditions of a light/dark cycle ( 12 h : 12 h ) .
	manualset3
108512	7	402904	5	NULL	NULL	0	NULL	biological rhythms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice fed with a 2.0 % GF-containing diet ( GF2 .0 ) transiently exhibited phase advance or phase advance-like phenomenon by 1-3 h in terms of the biological rhythms of T ( b ) or LA , respectively ( both , P & lt ; 0.05 ) while mice were kept under conditions of a light/dark cycle ( 12 h : 12 h ) .
	manualset3
108513	8	402904	5	NULL	NULL	NULL	NULL	T ( b )	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mice fed with a 2.0 % GF-containing diet ( GF2 .0 ) transiently exhibited phase advance or phase advance-like phenomenon by 1-3 h in terms of the biological rhythms of T ( b ) or LA , respectively ( both , P & lt ; 0.05 ) while mice were kept under conditions of a light/dark cycle ( 12 h : 12 h ) .
	manualset3
108514	9	402904	5	NULL	NULL	0	NULL	LA	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice fed with a 2.0 % GF-containing diet ( GF2 .0 ) transiently exhibited phase advance or phase advance-like phenomenon by 1-3 h in terms of the biological rhythms of T ( b ) or LA , respectively ( both , P & lt ; 0.05 ) while mice were kept under conditions of a light/dark cycle ( 12 h : 12 h ) .
	manualset3
108515	10	402904	5	NULL	NULL	0	NULL	P & lt ; 0.05 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice fed with a 2.0 % GF-containing diet ( GF2 .0 ) transiently exhibited phase advance or phase advance-like phenomenon by 1-3 h in terms of the biological rhythms of T ( b ) or LA , respectively ( both , P & lt ; 0.05 ) while mice were kept under conditions of a light/dark cycle ( 12 h : 12 h ) .
	manualset3
108516	11	402904	5	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice fed with a 2.0 % GF-containing diet ( GF2 .0 ) transiently exhibited phase advance or phase advance-like phenomenon by 1-3 h in terms of the biological rhythms of T ( b ) or LA , respectively ( both , P & lt ; 0.05 ) while mice were kept under conditions of a light/dark cycle ( 12 h : 12 h ) .
	manualset3
108517	12	402904	5	NULL	NULL	0	NULL	conditions of a light/dark cycle	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice fed with a 2.0 % GF-containing diet ( GF2 .0 ) transiently exhibited phase advance or phase advance-like phenomenon by 1-3 h in terms of the biological rhythms of T ( b ) or LA , respectively ( both , P & lt ; 0.05 ) while mice were kept under conditions of a light/dark cycle ( 12 h : 12 h ) .
	manualset3
108518	13	402904	5	NULL	NULL	0	NULL	12 h : 12 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice fed with a 2.0 % GF-containing diet ( GF2 .0 ) transiently exhibited phase advance or phase advance-like phenomenon by 1-3 h in terms of the biological rhythms of T ( b ) or LA , respectively ( both , P & lt ; 0.05 ) while mice were kept under conditions of a light/dark cycle ( 12 h : 12 h ) .
	manualset3
108519	1	402905	5	NULL	NULL	0	NULL	cascade 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A cascade of interactions follows , mediating embryo migration across the epithelium .
	manualset3
108520	2	402905	5	NULL	NULL	0	NULL	interactions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A cascade of interactions follows , mediating embryo migration across the epithelium .
	manualset3
108521	3	402905	5	NULL	NULL	0	NULL	embryo migration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A cascade of interactions follows , mediating embryo migration across the epithelium .
	manualset3
108522	4	402905	5	NULL	NULL	0	NULL	epithelium 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	A cascade of interactions follows , mediating embryo migration across the epithelium .
	manualset3
108523	1	402906	5	NULL	NULL	0	NULL	Mice homozygous for the spastic mutation ( spa )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice homozygous for the spastic mutation ( spa ) suffer from a complex motor disorder resulting from reduced CNS levels of the adult glycine receptor isoform GlyRA , which is composed of ligand-binding alpha 1 and structural beta polypeptides .
	manualset3
108524	2	402906	5	NULL	NULL	0	NULL	complex motor disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice homozygous for the spastic mutation ( spa ) suffer from a complex motor disorder resulting from reduced CNS levels of the adult glycine receptor isoform GlyRA , which is composed of ligand-binding alpha 1 and structural beta polypeptides .
	manualset3
108525	3	402906	5	NULL	NULL	0	NULL	CNS levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice homozygous for the spastic mutation ( spa ) suffer from a complex motor disorder resulting from reduced CNS levels of the adult glycine receptor isoform GlyRA , which is composed of ligand-binding alpha 1 and structural beta polypeptides .
	manualset3
108526	4	402906	5	NULL	NULL	0	NULL	adult glycine receptor isoform GlyRA 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice homozygous for the spastic mutation ( spa ) suffer from a complex motor disorder resulting from reduced CNS levels of the adult glycine receptor isoform GlyRA , which is composed of ligand-binding alpha 1 and structural beta polypeptides .
	manualset3
108527	5	402906	5	NULL	NULL	0	NULL	ligand-binding alpha 1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice homozygous for the spastic mutation ( spa ) suffer from a complex motor disorder resulting from reduced CNS levels of the adult glycine receptor isoform GlyRA , which is composed of ligand-binding alpha 1 and structural beta polypeptides .
	manualset3
108528	6	402906	5	NULL	NULL	0	NULL	structural beta polypeptides	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice homozygous for the spastic mutation ( spa ) suffer from a complex motor disorder resulting from reduced CNS levels of the adult glycine receptor isoform GlyRA , which is composed of ligand-binding alpha 1 and structural beta polypeptides .
	manualset3
108529	1	402907	5	NULL	NULL	0	NULL	Mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice maintained on a diet containing 0.75 % BHA for 8 days showed a 50 % reduction in maximal ODC induction following treatment with TPA when compared to mice fed a control diet .
	manualset3
108530	2	402907	5	NULL	NULL	0	NULL	diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice maintained on a diet containing 0.75 % BHA for 8 days showed a 50 % reduction in maximal ODC induction following treatment with TPA when compared to mice fed a control diet .
	manualset3
108531	3	402907	5	NULL	NULL	0	NULL	0.75 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice maintained on a diet containing 0.75 % BHA for 8 days showed a 50 % reduction in maximal ODC induction following treatment with TPA when compared to mice fed a control diet .
	manualset3
108532	4	402907	5	NULL	NULL	0	NULL	BHA	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice maintained on a diet containing 0.75 % BHA for 8 days showed a 50 % reduction in maximal ODC induction following treatment with TPA when compared to mice fed a control diet .
	manualset3
108533	5	402907	5	NULL	NULL	0	NULL	8 days	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice maintained on a diet containing 0.75 % BHA for 8 days showed a 50 % reduction in maximal ODC induction following treatment with TPA when compared to mice fed a control diet .
	manualset3
108534	6	402907	5	NULL	NULL	0	NULL	50 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice maintained on a diet containing 0.75 % BHA for 8 days showed a 50 % reduction in maximal ODC induction following treatment with TPA when compared to mice fed a control diet .
	manualset3
108535	7	402907	5	NULL	NULL	0	NULL	maximal ODC induction	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice maintained on a diet containing 0.75 % BHA for 8 days showed a 50 % reduction in maximal ODC induction following treatment with TPA when compared to mice fed a control diet .
	manualset3
108536	8	402907	5	NULL	NULL	0	NULL	treatment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice maintained on a diet containing 0.75 % BHA for 8 days showed a 50 % reduction in maximal ODC induction following treatment with TPA when compared to mice fed a control diet .
	manualset3
108537	9	402907	5	NULL	NULL	0	NULL	TPA	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice maintained on a diet containing 0.75 % BHA for 8 days showed a 50 % reduction in maximal ODC induction following treatment with TPA when compared to mice fed a control diet .
	manualset3
108538	10	402907	5	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice maintained on a diet containing 0.75 % BHA for 8 days showed a 50 % reduction in maximal ODC induction following treatment with TPA when compared to mice fed a control diet .
	manualset3
108539	11	402907	5	NULL	NULL	0	NULL	control diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice maintained on a diet containing 0.75 % BHA for 8 days showed a 50 % reduction in maximal ODC induction following treatment with TPA when compared to mice fed a control diet .
	manualset3
108540	1	402908	5	NULL	NULL	0	NULL	Mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice with IFN-gamma receptor deficiency are less susceptible to experimental autoimmune myasthenia gravis .
	manualset3
108541	2	402908	5	NULL	NULL	0	NULL	IFN-gamma receptor deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice with IFN-gamma receptor deficiency are less susceptible to experimental autoimmune myasthenia gravis .
	manualset3
108542	3	402908	5	NULL	NULL	0	NULL	experimental autoimmune myasthenia gravis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice with IFN-gamma receptor deficiency are less susceptible to experimental autoimmune myasthenia gravis .
	manualset3
108543	1	402909	5	NULL	NULL	0	NULL	Mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice with beta cell overexpression of glycogen synthase kinase-3beta have reduced beta cell mass and proliferation .
	manualset3
108544	2	402909	5	NULL	NULL	NULL	NULL	beta cell	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mice with beta cell overexpression of glycogen synthase kinase-3beta have reduced beta cell mass and proliferation .
	manualset3
108545	3	402909	5	NULL	NULL	0	NULL	overexpression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice with beta cell overexpression of glycogen synthase kinase-3beta have reduced beta cell mass and proliferation .
	manualset3
108546	4	402909	5	NULL	NULL	0	NULL	glycogen synthase kinase-3beta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice with beta cell overexpression of glycogen synthase kinase-3beta have reduced beta cell mass and proliferation .
	manualset3
108547	5	402909	5	NULL	NULL	0	NULL	beta cell mass	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice with beta cell overexpression of glycogen synthase kinase-3beta have reduced beta cell mass and proliferation .
	manualset3
108548	6	402909	5	NULL	NULL	0	NULL	proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice with beta cell overexpression of glycogen synthase kinase-3beta have reduced beta cell mass and proliferation .
	manualset3
108549	1	402910	5	NULL	NULL	0	NULL	Mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice with established 100-mm3 s.c. tumors who received one intratumoral injection of antibody 38C2 followed by systemic i.p. injections with the etoposide prodrug showed a 75 % reduction in s.c. tumor growth .
	manualset3
108550	2	402910	5	NULL	NULL	0	NULL	100-mm3	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice with established 100-mm3 s.c. tumors who received one intratumoral injection of antibody 38C2 followed by systemic i.p. injections with the etoposide prodrug showed a 75 % reduction in s.c. tumor growth .
	manualset3
108551	3	402910	5	NULL	NULL	0	NULL	s.c. tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice with established 100-mm3 s.c. tumors who received one intratumoral injection of antibody 38C2 followed by systemic i.p. injections with the etoposide prodrug showed a 75 % reduction in s.c. tumor growth .
	manualset3
108552	4	402910	5	NULL	NULL	0	NULL	intratumoral injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice with established 100-mm3 s.c. tumors who received one intratumoral injection of antibody 38C2 followed by systemic i.p. injections with the etoposide prodrug showed a 75 % reduction in s.c. tumor growth .
	manualset3
108553	5	402910	5	NULL	NULL	0	NULL	antibody 38C2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice with established 100-mm3 s.c. tumors who received one intratumoral injection of antibody 38C2 followed by systemic i.p. injections with the etoposide prodrug showed a 75 % reduction in s.c. tumor growth .
	manualset3
108554	6	402910	5	NULL	NULL	0	NULL	systemic i.p. injections	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice with established 100-mm3 s.c. tumors who received one intratumoral injection of antibody 38C2 followed by systemic i.p. injections with the etoposide prodrug showed a 75 % reduction in s.c. tumor growth .
	manualset3
108555	7	402910	5	NULL	NULL	0	NULL	etoposide prodrug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice with established 100-mm3 s.c. tumors who received one intratumoral injection of antibody 38C2 followed by systemic i.p. injections with the etoposide prodrug showed a 75 % reduction in s.c. tumor growth .
	manualset3
108556	8	402910	5	NULL	NULL	0	NULL	75 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice with established 100-mm3 s.c. tumors who received one intratumoral injection of antibody 38C2 followed by systemic i.p. injections with the etoposide prodrug showed a 75 % reduction in s.c. tumor growth .
	manualset3
108557	9	402910	5	NULL	NULL	0	NULL	reduction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice with established 100-mm3 s.c. tumors who received one intratumoral injection of antibody 38C2 followed by systemic i.p. injections with the etoposide prodrug showed a 75 % reduction in s.c. tumor growth .
	manualset3
108558	10	402910	5	NULL	NULL	0	NULL	s.c. tumor growth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice with established 100-mm3 s.c. tumors who received one intratumoral injection of antibody 38C2 followed by systemic i.p. injections with the etoposide prodrug showed a 75 % reduction in s.c. tumor growth .
	manualset3
108559	1	402911	5	NULL	NULL	0	NULL	MicroRNA-200b	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	MicroRNA-200b regulates vascular endothelial growth factor-mediated alterations in diabetic retinopathy .
	manualset3
108560	2	402911	5	NULL	NULL	0	NULL	vascular endothelial growth factor-mediated alterations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MicroRNA-200b regulates vascular endothelial growth factor-mediated alterations in diabetic retinopathy .
	manualset3
108561	3	402911	5	NULL	NULL	0	NULL	diabetic retinopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	MicroRNA-200b regulates vascular endothelial growth factor-mediated alterations in diabetic retinopathy .
	manualset3
108562	1	402912	5	NULL	NULL	0	NULL	MicroRNA-200c ( miR-200c )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	MicroRNA-200c ( miR-200c ) has been shown to suppress epithelial-mesenchymal transition ( EMT ) , which is attributed mainly to targeting of ZEB1/ZEB2 , repressors of the cell-cell contact protein E-cadherin .
	manualset3
108563	2	402912	5	NULL	NULL	0	NULL	epithelial-mesenchymal transition ( EMT )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MicroRNA-200c ( miR-200c ) has been shown to suppress epithelial-mesenchymal transition ( EMT ) , which is attributed mainly to targeting of ZEB1/ZEB2 , repressors of the cell-cell contact protein E-cadherin .
	manualset3
108564	3	402912	5	NULL	NULL	0	NULL	ZEB1/ZEB2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	MicroRNA-200c ( miR-200c ) has been shown to suppress epithelial-mesenchymal transition ( EMT ) , which is attributed mainly to targeting of ZEB1/ZEB2 , repressors of the cell-cell contact protein E-cadherin .
	manualset3
108565	4	402912	5	NULL	NULL	0	NULL	repressors of the cell-cell contact protein E-cadherin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	MicroRNA-200c ( miR-200c ) has been shown to suppress epithelial-mesenchymal transition ( EMT ) , which is attributed mainly to targeting of ZEB1/ZEB2 , repressors of the cell-cell contact protein E-cadherin .
	manualset3
108566	1	402913	5	NULL	NULL	0	NULL	case	person												NULL		0	NULL	NULL	NULL	NULL	NULL	A case acute intermittent porphyria is described in which the inappropriate antidiuretic hormone secretion syndrome developed masked by rapidly increasing sensorimotor polyneuropathy .
	manualset3
108567	2	402913	5	NULL	NULL	0	NULL	acute intermittent porphyria	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A case acute intermittent porphyria is described in which the inappropriate antidiuretic hormone secretion syndrome developed masked by rapidly increasing sensorimotor polyneuropathy .
	manualset3
108568	3	402913	5	NULL	NULL	0	NULL	inappropriate antidiuretic hormone secretion syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A case acute intermittent porphyria is described in which the inappropriate antidiuretic hormone secretion syndrome developed masked by rapidly increasing sensorimotor polyneuropathy .
	manualset3
108569	4	402913	5	NULL	NULL	0	NULL	sensorimotor polyneuropathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A case acute intermittent porphyria is described in which the inappropriate antidiuretic hormone secretion syndrome developed masked by rapidly increasing sensorimotor polyneuropathy .
	manualset3
108570	1	402914	5	NULL	NULL	0	NULL	MicroRNA ( miRNA )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	MicroRNA ( miRNA ) play important roles in tumorigenesis and drug sensitivity .
	manualset3
108571	2	402914	5	NULL	NULL	0	NULL	 important roles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MicroRNA ( miRNA ) play important roles in tumorigenesis and drug sensitivity .
	manualset3
108572	3	402914	5	NULL	NULL	0	NULL	tumorigenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MicroRNA ( miRNA ) play important roles in tumorigenesis and drug sensitivity .
	manualset3
108573	4	402914	5	NULL	NULL	0	NULL	drug sensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MicroRNA ( miRNA ) play important roles in tumorigenesis and drug sensitivity .
	manualset3
108574	1	402915	5	NULL	NULL	0	NULL	MicroRNA Modulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MicroRNA Modulation in Obesity and Periodontitis .
	manualset3
108575	2	402915	5	NULL	NULL	0	NULL	Obesity	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	MicroRNA Modulation in Obesity and Periodontitis .
	manualset3
108576	3	402915	5	NULL	NULL	0	NULL	Periodontitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	MicroRNA Modulation in Obesity and Periodontitis .
	manualset3
108577	1	402916	5	NULL	NULL	0	NULL	MicroRNAs ( miRNAs )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	MicroRNAs ( miRNAs ) made up the large majority of small RNAs , and we identified over 400 different cellular pre-miRNAs .
	manualset3
108578	2	402916	5	NULL	NULL	0	NULL	small RNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	MicroRNAs ( miRNAs ) made up the large majority of small RNAs , and we identified over 400 different cellular pre-miRNAs .
	manualset3
108579	3	402916	5	NULL	NULL	0	NULL	400	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	MicroRNAs ( miRNAs ) made up the large majority of small RNAs , and we identified over 400 different cellular pre-miRNAs .
	manualset3
108580	4	402916	5	NULL	NULL	0	NULL	cellular pre-miRNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	MicroRNAs ( miRNAs ) made up the large majority of small RNAs , and we identified over 400 different cellular pre-miRNAs .
	manualset3
108581	1	402917	5	NULL	NULL	0	NULL	MicroRNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	MicroRNAs are critical regulators of endothelial cell differentiation and ischaemia-induced neovascularization .
	manualset3
108582	2	402917	5	NULL	NULL	0	NULL	critical regulators	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	MicroRNAs are critical regulators of endothelial cell differentiation and ischaemia-induced neovascularization .
	manualset3
108583	3	402917	5	NULL	NULL	0	NULL	endothelial cell differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MicroRNAs are critical regulators of endothelial cell differentiation and ischaemia-induced neovascularization .
	manualset3
108584	4	402917	5	NULL	NULL	0	NULL	ischaemia-induced neovascularization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MicroRNAs are critical regulators of endothelial cell differentiation and ischaemia-induced neovascularization .
	manualset3
108585	1	402918	5	NULL	NULL	0	NULL	Microarray analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Microarray analysis of yeast cells treated with sublethal concentrations of chitosan revealed induction of the environmental stress response and three more major transcriptional responses .
	manualset3
108586	2	402918	5	NULL	NULL	0	NULL	yeast cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Microarray analysis of yeast cells treated with sublethal concentrations of chitosan revealed induction of the environmental stress response and three more major transcriptional responses .
	manualset3
108587	3	402918	5	NULL	NULL	0	NULL	sublethal concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Microarray analysis of yeast cells treated with sublethal concentrations of chitosan revealed induction of the environmental stress response and three more major transcriptional responses .
	manualset3
108588	4	402918	5	NULL	NULL	0	NULL	chitosan	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Microarray analysis of yeast cells treated with sublethal concentrations of chitosan revealed induction of the environmental stress response and three more major transcriptional responses .
	manualset3
108589	5	402918	5	NULL	NULL	0	NULL	induction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Microarray analysis of yeast cells treated with sublethal concentrations of chitosan revealed induction of the environmental stress response and three more major transcriptional responses .
	manualset3
108590	6	402918	5	NULL	NULL	0	NULL	environmental stress response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Microarray analysis of yeast cells treated with sublethal concentrations of chitosan revealed induction of the environmental stress response and three more major transcriptional responses .
	manualset3
108591	7	402918	5	NULL	NULL	0	NULL	transcriptional responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Microarray analysis of yeast cells treated with sublethal concentrations of chitosan revealed induction of the environmental stress response and three more major transcriptional responses .
	manualset3
108592	1	402919	5	NULL	NULL	0	NULL	Microarray technology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Microarray technology is increasingly used for a miniaturised and parallel measurement of binding constants .
	manualset3
108593	2	402919	5	NULL	NULL	0	NULL	miniaturised and parallel measurement	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Microarray technology is increasingly used for a miniaturised and parallel measurement of binding constants .
	manualset3
108594	3	402919	5	NULL	NULL	0	NULL	binding constants	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Microarray technology is increasingly used for a miniaturised and parallel measurement of binding constants .
	manualset3
108595	1	402920	5	NULL	NULL	0	NULL	Microarrays	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Microarrays identified a set of miRNA that were induced by culture conditions and potentially able to bind to the BCL2 3 ' - UTR .
	manualset3
108596	2	402920	5	NULL	NULL	0	NULL	miRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Microarrays identified a set of miRNA that were induced by culture conditions and potentially able to bind to the BCL2 3 ' - UTR .
	manualset3
108597	3	402920	5	NULL	NULL	0	NULL	culture conditions	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Microarrays identified a set of miRNA that were induced by culture conditions and potentially able to bind to the BCL2 3 ' - UTR .
	manualset3
108598	4	402920	5	NULL	NULL	0	NULL	BCL2 3 ' - UTR	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Microarrays identified a set of miRNA that were induced by culture conditions and potentially able to bind to the BCL2 3 ' - UTR .
	manualset3
108599	1	402921	5	NULL	NULL	0	NULL	case example	person												NULL		0	NULL	NULL	NULL	NULL	NULL	A case example from the Mental Health and Poverty Project in sub-Saharan Africa illustrates how this approach can be put into practice-in particular , by focusing upon training in core transferrable research skills .
	manualset3
108600	2	402921	5	NULL	NULL	0	NULL	Mental Health and Poverty Project	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A case example from the Mental Health and Poverty Project in sub-Saharan Africa illustrates how this approach can be put into practice-in particular , by focusing upon training in core transferrable research skills .
	manualset3
108601	3	402921	5	NULL	NULL	0	NULL	sub-Saharan Africa	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A case example from the Mental Health and Poverty Project in sub-Saharan Africa illustrates how this approach can be put into practice-in particular , by focusing upon training in core transferrable research skills .
	manualset3
108602	4	402921	5	NULL	NULL	0	NULL	approach 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A case example from the Mental Health and Poverty Project in sub-Saharan Africa illustrates how this approach can be put into practice-in particular , by focusing upon training in core transferrable research skills .
	manualset3
108603	5	402921	5	NULL	NULL	0	NULL	core transferrable research skills	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A case example from the Mental Health and Poverty Project in sub-Saharan Africa illustrates how this approach can be put into practice-in particular , by focusing upon training in core transferrable research skills .
	manualset3
108604	1	402922	5	NULL	NULL	0	NULL	Microbial diversity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Microbial diversity was assessed to species level for samples from the latter three subject groups .
	manualset3
108605	2	402922	5	NULL	NULL	0	NULL	species level	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Microbial diversity was assessed to species level for samples from the latter three subject groups .
	manualset3
108606	3	402922	5	NULL	NULL	0	NULL	samples 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Microbial diversity was assessed to species level for samples from the latter three subject groups .
	manualset3
108607	4	402922	5	NULL	NULL	0	NULL	latter three subject groups 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Microbial diversity was assessed to species level for samples from the latter three subject groups .
	manualset3
108608	1	402923	5	NULL	NULL	0	NULL	Microbial treatment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Microbial treatment of environmental pollutants including dyes with white rot fungi has received wide attention as a potential alternative for conventional methods in wastewater treatment .
	manualset3
108609	2	402923	5	NULL	NULL	0	NULL	environmental pollutants	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Microbial treatment of environmental pollutants including dyes with white rot fungi has received wide attention as a potential alternative for conventional methods in wastewater treatment .
	manualset3
108610	3	402923	5	NULL	NULL	0	NULL	dyes 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Microbial treatment of environmental pollutants including dyes with white rot fungi has received wide attention as a potential alternative for conventional methods in wastewater treatment .
	manualset3
108611	4	402923	5	NULL	NULL	0	NULL	white rot fungi 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Microbial treatment of environmental pollutants including dyes with white rot fungi has received wide attention as a potential alternative for conventional methods in wastewater treatment .
	manualset3
108612	5	402923	5	NULL	NULL	0	NULL	wide attention	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Microbial treatment of environmental pollutants including dyes with white rot fungi has received wide attention as a potential alternative for conventional methods in wastewater treatment .
	manualset3
108613	6	402923	5	NULL	NULL	0	NULL	conventional methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Microbial treatment of environmental pollutants including dyes with white rot fungi has received wide attention as a potential alternative for conventional methods in wastewater treatment .
	manualset3
108614	7	402923	5	NULL	NULL	0	NULL	wastewater treatment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Microbial treatment of environmental pollutants including dyes with white rot fungi has received wide attention as a potential alternative for conventional methods in wastewater treatment .
	manualset3
108615	1	402924	5	NULL	NULL	0	NULL	Microbiology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Microbiology and previously reported cases of infections by this organism are reviewed .
	manualset3
108616	2	402924	5	NULL	NULL	0	NULL	previously reported cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Microbiology and previously reported cases of infections by this organism are reviewed .
	manualset3
108617	3	402924	5	NULL	NULL	0	NULL	infections 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Microbiology and previously reported cases of infections by this organism are reviewed .
	manualset3
108618	4	402924	5	NULL	NULL	0	NULL	organism 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Microbiology and previously reported cases of infections by this organism are reviewed .
	manualset3
108619	1	402925	5	NULL	NULL	0	NULL	Microcaudate cercariae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Microcaudate cercariae emerge from this snail and develop into unencysted metacercariae in the kidney of second intermediate host snails H. ( C. ) aspersa and Otala punctata ( natural hosts ) and Theba pisana ( experimental host ) .
	manualset3
108620	2	402925	5	NULL	NULL	0	NULL	snail 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Microcaudate cercariae emerge from this snail and develop into unencysted metacercariae in the kidney of second intermediate host snails H. ( C. ) aspersa and Otala punctata ( natural hosts ) and Theba pisana ( experimental host ) .
	manualset3
108621	3	402925	5	NULL	NULL	0	NULL	unencysted metacercariae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Microcaudate cercariae emerge from this snail and develop into unencysted metacercariae in the kidney of second intermediate host snails H. ( C. ) aspersa and Otala punctata ( natural hosts ) and Theba pisana ( experimental host ) .
	manualset3
108622	4	402925	5	NULL	NULL	0	NULL	kidney 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Microcaudate cercariae emerge from this snail and develop into unencysted metacercariae in the kidney of second intermediate host snails H. ( C. ) aspersa and Otala punctata ( natural hosts ) and Theba pisana ( experimental host ) .
	manualset3
108623	5	402925	5	NULL	NULL	0	NULL	second intermediate host snails H. ( C. ) aspersa	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Microcaudate cercariae emerge from this snail and develop into unencysted metacercariae in the kidney of second intermediate host snails H. ( C. ) aspersa and Otala punctata ( natural hosts ) and Theba pisana ( experimental host ) .
	manualset3
108624	6	402925	5	NULL	NULL	0	NULL	Otala punctata ( natural hosts )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Microcaudate cercariae emerge from this snail and develop into unencysted metacercariae in the kidney of second intermediate host snails H. ( C. ) aspersa and Otala punctata ( natural hosts ) and Theba pisana ( experimental host ) .
	manualset3
108625	7	402925	5	NULL	NULL	0	NULL	Theba pisana ( experimental host )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Microcaudate cercariae emerge from this snail and develop into unencysted metacercariae in the kidney of second intermediate host snails H. ( C. ) aspersa and Otala punctata ( natural hosts ) and Theba pisana ( experimental host ) .
	manualset3
108626	1	402926	5	NULL	NULL	0	NULL	Microdialysis assessment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Microdialysis assessment of adipose tissue metabolism in post-absorptive obese NIDDM subjects .
	manualset3
108627	2	402926	5	NULL	NULL	0	NULL	adipose tissue metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Microdialysis assessment of adipose tissue metabolism in post-absorptive obese NIDDM subjects .
	manualset3
112974	3	402926	5	NULL	NULL	0	NULL	post-absorptive obese NIDDM subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Microdialysis assessment of adipose tissue metabolism in post-absorptive obese NIDDM subjects .
	manualset3
108628	1	402927	5	NULL	NULL	0	NULL	Microfilament bundles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Microfilament bundles in RAB5A gene over-expressed AGZY83-a cells were shown to be denser than in control cells using confocal laser scanning microscope ( CLSM ) .
	manualset3
108629	2	402927	5	NULL	NULL	0	NULL	RAB5A gene over-expressed AGZY83-a cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Microfilament bundles in RAB5A gene over-expressed AGZY83-a cells were shown to be denser than in control cells using confocal laser scanning microscope ( CLSM ) .
	manualset3
108630	3	402927	5	NULL	NULL	0	NULL	control cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Microfilament bundles in RAB5A gene over-expressed AGZY83-a cells were shown to be denser than in control cells using confocal laser scanning microscope ( CLSM ) .
	manualset3
108631	4	402927	5	NULL	NULL	0	NULL	confocal laser scanning microscope ( CLSM )	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Microfilament bundles in RAB5A gene over-expressed AGZY83-a cells were shown to be denser than in control cells using confocal laser scanning microscope ( CLSM ) .
	manualset3
108632	1	402928	5	NULL	NULL	0	NULL	Microglia	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Microglia subjected to oxygen-glucose deprivation died via necrosis .
	manualset3
108633	2	402928	5	NULL	NULL	NULL	NULL	oxygen-glucose deprivation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Microglia subjected to oxygen-glucose deprivation died via necrosis .
	manualset3
108634	3	402928	5	NULL	NULL	0	NULL	necrosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Microglia subjected to oxygen-glucose deprivation died via necrosis .
	manualset3
108635	1	402929	5	NULL	NULL	0	NULL	Microgravimetric technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Microgravimetric technique was used to measure the water content of tumors and adjacent brain .
	manualset3
108637	2	402929	5	NULL	NULL	NULL	NULL	water content	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Microgravimetric technique was used to measure the water content of tumors and adjacent brain .
	manualset3
108638	3	402929	5	NULL	NULL	NULL	NULL	tumors 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Microgravimetric technique was used to measure the water content of tumors and adjacent brain .
	manualset3
108639	4	402929	5	NULL	NULL	NULL	NULL	adjacent brain	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Microgravimetric technique was used to measure the water content of tumors and adjacent brain .
	manualset3
108640	1	402930	5	NULL	NULL	0	NULL	Microinfusion 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Microinfusion of AP5 into the medial septum significantly lowered power of tail pinch-induced theta but did not affect frequency .
	manualset3
108641	2	402930	5	NULL	NULL	0	NULL	AP5	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Microinfusion of AP5 into the medial septum significantly lowered power of tail pinch-induced theta but did not affect frequency .
	manualset3
108642	3	402930	5	NULL	NULL	0	NULL	medial septum	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Microinfusion of AP5 into the medial septum significantly lowered power of tail pinch-induced theta but did not affect frequency .
	manualset3
108643	4	402930	5	NULL	NULL	0	NULL	power 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Microinfusion of AP5 into the medial septum significantly lowered power of tail pinch-induced theta but did not affect frequency .
	manualset3
108644	5	402930	5	NULL	NULL	0	NULL	tail pinch-induced theta 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Microinfusion of AP5 into the medial septum significantly lowered power of tail pinch-induced theta but did not affect frequency .
	manualset3
108645	6	402930	5	NULL	NULL	0	NULL	frequency 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Microinfusion of AP5 into the medial septum significantly lowered power of tail pinch-induced theta but did not affect frequency .
	manualset3
108646	1	402931	5	NULL	NULL	0	NULL	Behavior 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Behavior of blood coagulation factors in icterogenic viral hepatitis ) .
	manualset3
108647	2	402931	5	NULL	NULL	0	NULL	blood coagulation factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Behavior of blood coagulation factors in icterogenic viral hepatitis ) .
	manualset3
108648	3	402931	5	NULL	NULL	0	NULL	icterogenic viral hepatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Behavior of blood coagulation factors in icterogenic viral hepatitis ) .
	manualset3
108649	1	402932	5	NULL	NULL	0	NULL	Microiontophoresis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Microiontophoresis of alpha-CGRP excited seven of 17 tested neurons .
	manualset3
108650	2	402932	5	NULL	NULL	0	NULL	alpha-CGRP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Microiontophoresis of alpha-CGRP excited seven of 17 tested neurons .
	manualset3
108651	3	402932	5	NULL	NULL	NULL	NULL	seven of 17 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Microiontophoresis of alpha-CGRP excited seven of 17 tested neurons .
	manualset3
108652	4	402932	5	NULL	NULL	0	NULL	tested neurons 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Microiontophoresis of alpha-CGRP excited seven of 17 tested neurons .
	manualset3
108653	1	402933	5	NULL	NULL	0	NULL	Micronised sodium lauryl sulphate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Micronised sodium lauryl sulphate added to the mixture was more effective in de-agglomeration than equivalent concentrations in the dissolution media .
	manualset3
108654	2	402933	5	NULL	NULL	0	NULL	mixture 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Micronised sodium lauryl sulphate added to the mixture was more effective in de-agglomeration than equivalent concentrations in the dissolution media .
	manualset3
108655	3	402933	5	NULL	NULL	0	NULL	de-agglomeration	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Micronised sodium lauryl sulphate added to the mixture was more effective in de-agglomeration than equivalent concentrations in the dissolution media .
	manualset3
108656	4	402933	5	NULL	NULL	0	NULL	equivalent concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Micronised sodium lauryl sulphate added to the mixture was more effective in de-agglomeration than equivalent concentrations in the dissolution media .
	manualset3
108657	5	402933	5	NULL	NULL	0	NULL	dissolution media 	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Micronised sodium lauryl sulphate added to the mixture was more effective in de-agglomeration than equivalent concentrations in the dissolution media .
	manualset3
108658	1	402934	5	NULL	NULL	0	NULL	Micronutrients 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Micronutrients and human cancer risks -- prospects for prevention .
	manualset3
108659	2	402934	5	NULL	NULL	0	NULL	human	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Micronutrients and human cancer risks -- prospects for prevention .
	manualset3
108660	3	402934	5	NULL	NULL	0	NULL	cancer risks	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Micronutrients and human cancer risks -- prospects for prevention .
	manualset3
108661	4	402934	5	NULL	NULL	0	NULL	prospects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Micronutrients and human cancer risks -- prospects for prevention .
	manualset3
108662	5	402934	5	NULL	NULL	0	NULL	prevention 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Micronutrients and human cancer risks -- prospects for prevention .
	manualset3
108663	1	402935	5	NULL	NULL	0	NULL	Microsatellite markers	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Microsatellite markers are generally more polymorphic than other types of molecular markers such as allozymes or SNPs because the insertions/deletions that give rise to microsatellite variability are relatively common compared to nucleotide substitutions .
	manualset3
108664	2	402935	5	NULL	NULL	0	NULL	molecular markers	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Microsatellite markers are generally more polymorphic than other types of molecular markers such as allozymes or SNPs because the insertions/deletions that give rise to microsatellite variability are relatively common compared to nucleotide substitutions .
	manualset3
108665	3	402935	5	NULL	NULL	0	NULL	allozymes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Microsatellite markers are generally more polymorphic than other types of molecular markers such as allozymes or SNPs because the insertions/deletions that give rise to microsatellite variability are relatively common compared to nucleotide substitutions .
	manualset3
108666	4	402935	5	NULL	NULL	0	NULL	SNPs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Microsatellite markers are generally more polymorphic than other types of molecular markers such as allozymes or SNPs because the insertions/deletions that give rise to microsatellite variability are relatively common compared to nucleotide substitutions .
	manualset3
108667	5	402935	5	NULL	NULL	0	NULL	insertions/deletions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Microsatellite markers are generally more polymorphic than other types of molecular markers such as allozymes or SNPs because the insertions/deletions that give rise to microsatellite variability are relatively common compared to nucleotide substitutions .
	manualset3
108669	6	402935	5	NULL	NULL	NULL	NULL	microsatellite variability	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Microsatellite markers are generally more polymorphic than other types of molecular markers such as allozymes or SNPs because the insertions/deletions that give rise to microsatellite variability are relatively common compared to nucleotide substitutions .
	manualset3
108670	7	402935	5	NULL	NULL	NULL	NULL	nucleotide substitutions	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Microsatellite markers are generally more polymorphic than other types of molecular markers such as allozymes or SNPs because the insertions/deletions that give rise to microsatellite variability are relatively common compared to nucleotide substitutions .
	manualset3
108671	1	402936	5	NULL	NULL	0	NULL	Microscopic areas	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Microscopic areas of dysplasia , carcinoma in situ , or early carcinoma showed areas of tumor lysis and an inflammatory infiltrate consisting of lymphocytes and histiocytes .
	manualset3
108672	2	402936	5	NULL	NULL	0	NULL	dysplasia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Microscopic areas of dysplasia , carcinoma in situ , or early carcinoma showed areas of tumor lysis and an inflammatory infiltrate consisting of lymphocytes and histiocytes .
	manualset3
108673	3	402936	5	NULL	NULL	0	NULL	carcinoma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Microscopic areas of dysplasia , carcinoma in situ , or early carcinoma showed areas of tumor lysis and an inflammatory infiltrate consisting of lymphocytes and histiocytes .
	manualset3
108674	4	402936	5	NULL	NULL	0	NULL	early carcinoma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Microscopic areas of dysplasia , carcinoma in situ , or early carcinoma showed areas of tumor lysis and an inflammatory infiltrate consisting of lymphocytes and histiocytes .
	manualset3
108675	5	402936	5	NULL	NULL	0	NULL	areas 	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Microscopic areas of dysplasia , carcinoma in situ , or early carcinoma showed areas of tumor lysis and an inflammatory infiltrate consisting of lymphocytes and histiocytes .
	manualset3
108676	6	402936	5	NULL	NULL	0	NULL	tumor lysis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Microscopic areas of dysplasia , carcinoma in situ , or early carcinoma showed areas of tumor lysis and an inflammatory infiltrate consisting of lymphocytes and histiocytes .
	manualset3
108677	7	402936	5	NULL	NULL	0	NULL	inflammatory infiltrate	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Microscopic areas of dysplasia , carcinoma in situ , or early carcinoma showed areas of tumor lysis and an inflammatory infiltrate consisting of lymphocytes and histiocytes .
	manualset3
108678	8	402936	5	NULL	NULL	0	NULL	lymphocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Microscopic areas of dysplasia , carcinoma in situ , or early carcinoma showed areas of tumor lysis and an inflammatory infiltrate consisting of lymphocytes and histiocytes .
	manualset3
108679	9	402936	5	NULL	NULL	0	NULL	histiocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Microscopic areas of dysplasia , carcinoma in situ , or early carcinoma showed areas of tumor lysis and an inflammatory infiltrate consisting of lymphocytes and histiocytes .
	manualset3
108680	1	402937	5	NULL	NULL	0	NULL	Microscopic colitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Microscopic colitis-a cause of chronic watery diarrhoea .
	manualset3
108681	2	402937	5	NULL	NULL	0	NULL	chronic watery diarrhoea	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Microscopic colitis-a cause of chronic watery diarrhoea .
	manualset3
108682	1	402938	5	NULL	NULL	0	NULL	case 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of Behet 's syndrome with supeior vena cava syndrome .
	manualset3
108683	2	402938	5	NULL	NULL	0	NULL	Behet 's syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of Behet 's syndrome with supeior vena cava syndrome .
	manualset3
108684	3	402938	5	NULL	NULL	0	NULL	supeior vena cava syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of Behet 's syndrome with supeior vena cava syndrome .
	manualset3
108685	1	402939	5	NULL	NULL	0	NULL	Microscopic examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Microscopic examination of the 6.5 cm mass showed well-defined , round , nests of tumor cells surrounded by a rim of collagen .
	manualset3
108686	2	402939	5	NULL	NULL	0	NULL	6.5 cm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Microscopic examination of the 6.5 cm mass showed well-defined , round , nests of tumor cells surrounded by a rim of collagen .
	manualset3
108687	3	402939	5	NULL	NULL	0	NULL	mass 	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Microscopic examination of the 6.5 cm mass showed well-defined , round , nests of tumor cells surrounded by a rim of collagen .
	manualset3
108688	4	402939	5	NULL	NULL	0	NULL	nests of tumor cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Microscopic examination of the 6.5 cm mass showed well-defined , round , nests of tumor cells surrounded by a rim of collagen .
	manualset3
108689	5	402939	5	NULL	NULL	0	NULL	rim	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Microscopic examination of the 6.5 cm mass showed well-defined , round , nests of tumor cells surrounded by a rim of collagen .
	manualset3
108690	6	402939	5	NULL	NULL	0	NULL	collagen 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Microscopic examination of the 6.5 cm mass showed well-defined , round , nests of tumor cells surrounded by a rim of collagen .
	manualset3
108691	1	402940	5	NULL	NULL	0	NULL	Microscopic model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Microscopic versus macroscopic biomass models in activated sludge systems .
	manualset3
108692	2	402940	5	NULL	NULL	0	NULL	macroscopic biomass models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Microscopic versus macroscopic biomass models in activated sludge systems .
	manualset3
108693	3	402940	5	NULL	NULL	0	NULL	activated sludge systems	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Microscopic versus macroscopic biomass models in activated sludge systems .
	manualset3
108694	1	402941	5	NULL	NULL	0	NULL	Microsomes 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Microsomes containing recombinant CYP3A4-OR from these cell lines were up to 50-times more active in testosterone 6 beta-hydroxylase activity than recombinant CYP3A4 expressed alone and supplemented with purified rabbit CYPOR .
	manualset3
108695	2	402941	5	NULL	NULL	0	NULL	recombinant CYP3A4-OR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Microsomes containing recombinant CYP3A4-OR from these cell lines were up to 50-times more active in testosterone 6 beta-hydroxylase activity than recombinant CYP3A4 expressed alone and supplemented with purified rabbit CYPOR .
	manualset3
108696	3	402941	5	NULL	NULL	0	NULL	cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Microsomes containing recombinant CYP3A4-OR from these cell lines were up to 50-times more active in testosterone 6 beta-hydroxylase activity than recombinant CYP3A4 expressed alone and supplemented with purified rabbit CYPOR .
	manualset3
108697	4	402941	5	NULL	NULL	0	NULL	50-times	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Microsomes containing recombinant CYP3A4-OR from these cell lines were up to 50-times more active in testosterone 6 beta-hydroxylase activity than recombinant CYP3A4 expressed alone and supplemented with purified rabbit CYPOR .
	manualset3
108698	5	402941	5	NULL	NULL	0	NULL	testosterone	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Microsomes containing recombinant CYP3A4-OR from these cell lines were up to 50-times more active in testosterone 6 beta-hydroxylase activity than recombinant CYP3A4 expressed alone and supplemented with purified rabbit CYPOR .
	manualset3
108699	6	402941	5	NULL	NULL	0	NULL	6 beta-hydroxylase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Microsomes containing recombinant CYP3A4-OR from these cell lines were up to 50-times more active in testosterone 6 beta-hydroxylase activity than recombinant CYP3A4 expressed alone and supplemented with purified rabbit CYPOR .
	manualset3
108700	7	402941	5	NULL	NULL	0	NULL	recombinant CYP3A4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Microsomes containing recombinant CYP3A4-OR from these cell lines were up to 50-times more active in testosterone 6 beta-hydroxylase activity than recombinant CYP3A4 expressed alone and supplemented with purified rabbit CYPOR .
	manualset3
108701	8	402941	5	NULL	NULL	0	NULL	purified rabbit CYPOR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Microsomes containing recombinant CYP3A4-OR from these cell lines were up to 50-times more active in testosterone 6 beta-hydroxylase activity than recombinant CYP3A4 expressed alone and supplemented with purified rabbit CYPOR .
	manualset3
108702	1	402942	5	NULL	NULL	0	NULL	Microsurgical excision	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Microsurgical excision of multiple clear cell meningiomas of the cauda equina : a case report .
	manualset3
108703	2	402942	5	NULL	NULL	0	NULL	multiple clear cell meningiomas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Microsurgical excision of multiple clear cell meningiomas of the cauda equina : a case report .
	manualset3
108704	3	402942	5	NULL	NULL	0	NULL	cauda equina	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Microsurgical excision of multiple clear cell meningiomas of the cauda equina : a case report .
	manualset3
108705	4	402942	5	NULL	NULL	0	NULL	case report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Microsurgical excision of multiple clear cell meningiomas of the cauda equina : a case report .
	manualset3
108706	1	402943	5	NULL	NULL	0	NULL	case 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of Epstein-Barr virus infection with neurological complications is described .
	manualset3
108707	2	402943	5	NULL	NULL	0	NULL	Epstein-Barr virus infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of Epstein-Barr virus infection with neurological complications is described .
	manualset3
108708	3	402943	5	NULL	NULL	0	NULL	neurological complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of Epstein-Barr virus infection with neurological complications is described .
	manualset3
108709	1	402944	5	NULL	NULL	0	NULL	Microtubule-stabilizing agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Microtubule-stabilizing agents such as hexylene glycol and D ( 2 ) O also inhibit secretion .
	manualset3
108710	2	402944	5	NULL	NULL	0	NULL	hexylene glycol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Microtubule-stabilizing agents such as hexylene glycol and D ( 2 ) O also inhibit secretion .
	manualset3
108711	3	402944	5	NULL	NULL	0	NULL	D ( 2 ) O	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Microtubule-stabilizing agents such as hexylene glycol and D ( 2 ) O also inhibit secretion .
	manualset3
108712	4	402944	5	NULL	NULL	0	NULL	secretion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Microtubule-stabilizing agents such as hexylene glycol and D ( 2 ) O also inhibit secretion .
	manualset3
108713	1	402945	5	NULL	NULL	0	NULL	Mid-vermal cerebellar sections	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mid-vermal cerebellar sections were stained with antibodies to calbindin-D28k ( to visualize Purkinje cells ) and vesicular glutamate transporter 2 ( VGluT2 , to visualize climbing fibers ) .
	manualset3
108714	2	402945	5	NULL	NULL	0	NULL	antibodies 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mid-vermal cerebellar sections were stained with antibodies to calbindin-D28k ( to visualize Purkinje cells ) and vesicular glutamate transporter 2 ( VGluT2 , to visualize climbing fibers ) .
	manualset3
108715	3	402945	5	NULL	NULL	0	NULL	calbindin-D28k	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mid-vermal cerebellar sections were stained with antibodies to calbindin-D28k ( to visualize Purkinje cells ) and vesicular glutamate transporter 2 ( VGluT2 , to visualize climbing fibers ) .
	manualset3
108716	4	402945	5	NULL	NULL	0	NULL	Purkinje cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mid-vermal cerebellar sections were stained with antibodies to calbindin-D28k ( to visualize Purkinje cells ) and vesicular glutamate transporter 2 ( VGluT2 , to visualize climbing fibers ) .
	manualset3
108717	5	402945	5	NULL	NULL	0	NULL	vesicular glutamate transporter 2 ( VGluT2 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mid-vermal cerebellar sections were stained with antibodies to calbindin-D28k ( to visualize Purkinje cells ) and vesicular glutamate transporter 2 ( VGluT2 , to visualize climbing fibers ) .
	manualset3
108718	6	402945	5	NULL	NULL	0	NULL	climbing fibers	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Mid-vermal cerebellar sections were stained with antibodies to calbindin-D28k ( to visualize Purkinje cells ) and vesicular glutamate transporter 2 ( VGluT2 , to visualize climbing fibers ) .
	manualset3
108719	1	402946	5	NULL	NULL	0	NULL	12-month-old	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Middle-aged ( 12-month-old ) female rats that were retired breeders were categorized as maintaining or declining reproductive function based upon their estrous cyclicity ( regular 4-5 day cycles ) , fertility ( & gt ; 60 % successful pregnancy ) , and fecundity ( & gt ; 10 pups/litter ) .
	manualset3
108720	2	402946	5	NULL	NULL	0	NULL	Middle-aged female rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Middle-aged ( 12-month-old ) female rats that were retired breeders were categorized as maintaining or declining reproductive function based upon their estrous cyclicity ( regular 4-5 day cycles ) , fertility ( & gt ; 60 % successful pregnancy ) , and fecundity ( & gt ; 10 pups/litter ) .
	manualset3
108721	3	402946	5	NULL	NULL	0	NULL	retired breeders	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Middle-aged ( 12-month-old ) female rats that were retired breeders were categorized as maintaining or declining reproductive function based upon their estrous cyclicity ( regular 4-5 day cycles ) , fertility ( & gt ; 60 % successful pregnancy ) , and fecundity ( & gt ; 10 pups/litter ) .
	manualset3
108722	4	402946	5	NULL	NULL	0	NULL	reproductive function 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Middle-aged ( 12-month-old ) female rats that were retired breeders were categorized as maintaining or declining reproductive function based upon their estrous cyclicity ( regular 4-5 day cycles ) , fertility ( & gt ; 60 % successful pregnancy ) , and fecundity ( & gt ; 10 pups/litter ) .
	manualset3
108723	5	402946	5	NULL	NULL	0	NULL	estrous cyclicity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Middle-aged ( 12-month-old ) female rats that were retired breeders were categorized as maintaining or declining reproductive function based upon their estrous cyclicity ( regular 4-5 day cycles ) , fertility ( & gt ; 60 % successful pregnancy ) , and fecundity ( & gt ; 10 pups/litter ) .
	manualset3
108724	6	402946	5	NULL	NULL	0	NULL	 regular 4-5 day cycles	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Middle-aged ( 12-month-old ) female rats that were retired breeders were categorized as maintaining or declining reproductive function based upon their estrous cyclicity ( regular 4-5 day cycles ) , fertility ( & gt ; 60 % successful pregnancy ) , and fecundity ( & gt ; 10 pups/litter ) .
	manualset3
108725	7	402946	5	NULL	NULL	0	NULL	fertility 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Middle-aged ( 12-month-old ) female rats that were retired breeders were categorized as maintaining or declining reproductive function based upon their estrous cyclicity ( regular 4-5 day cycles ) , fertility ( & gt ; 60 % successful pregnancy ) , and fecundity ( & gt ; 10 pups/litter ) .
	manualset3
108726	8	402946	5	NULL	NULL	0	NULL	 60 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Middle-aged ( 12-month-old ) female rats that were retired breeders were categorized as maintaining or declining reproductive function based upon their estrous cyclicity ( regular 4-5 day cycles ) , fertility ( & gt ; 60 % successful pregnancy ) , and fecundity ( & gt ; 10 pups/litter ) .
	manualset3
108727	9	402946	5	NULL	NULL	0	NULL	successful pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Middle-aged ( 12-month-old ) female rats that were retired breeders were categorized as maintaining or declining reproductive function based upon their estrous cyclicity ( regular 4-5 day cycles ) , fertility ( & gt ; 60 % successful pregnancy ) , and fecundity ( & gt ; 10 pups/litter ) .
	manualset3
108728	10	402946	5	NULL	NULL	0	NULL	fecundity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Middle-aged ( 12-month-old ) female rats that were retired breeders were categorized as maintaining or declining reproductive function based upon their estrous cyclicity ( regular 4-5 day cycles ) , fertility ( & gt ; 60 % successful pregnancy ) , and fecundity ( & gt ; 10 pups/litter ) .
	manualset3
108729	11	402946	5	NULL	NULL	0	NULL	10 pups/litter 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Middle-aged ( 12-month-old ) female rats that were retired breeders were categorized as maintaining or declining reproductive function based upon their estrous cyclicity ( regular 4-5 day cycles ) , fertility ( & gt ; 60 % successful pregnancy ) , and fecundity ( & gt ; 10 pups/litter ) .
	manualset3
108730	1	402947	5	NULL	NULL	0	NULL	Middle ear carcinoids 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Middle ear carcinoids have previously been approached as benign entities , lacking any capacity for metastasizing .
	manualset3
108731	2	402947	5	NULL	NULL	0	NULL	benign entities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Middle ear carcinoids have previously been approached as benign entities , lacking any capacity for metastasizing .
	manualset3
108732	3	402947	5	NULL	NULL	0	NULL	capacity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Middle ear carcinoids have previously been approached as benign entities , lacking any capacity for metastasizing .
	manualset3
108733	1	402948	5	NULL	NULL	0	NULL	Midluteal progesterone ( P )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Midluteal progesterone ( P ) and estradiol ( E2 ) were determined in 91 clip patients ; 21 normal worn and 27 tubal ligation cases served as controls .
	manualset3
108734	2	402948	5	NULL	NULL	0	NULL	estradiol ( E2 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Midluteal progesterone ( P ) and estradiol ( E2 ) were determined in 91 clip patients ; 21 normal worn and 27 tubal ligation cases served as controls .
	manualset3
108735	3	402948	5	NULL	NULL	0	NULL	91 clip patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Midluteal progesterone ( P ) and estradiol ( E2 ) were determined in 91 clip patients ; 21 normal worn and 27 tubal ligation cases served as controls .
	manualset3
108736	4	402948	5	NULL	NULL	0	NULL	21 normal worn	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Midluteal progesterone ( P ) and estradiol ( E2 ) were determined in 91 clip patients ; 21 normal worn and 27 tubal ligation cases served as controls .
	manualset3
108737	5	402948	5	NULL	NULL	0	NULL	27 tubal ligation cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Midluteal progesterone ( P ) and estradiol ( E2 ) were determined in 91 clip patients ; 21 normal worn and 27 tubal ligation cases served as controls .
	manualset3
108738	6	402948	5	NULL	NULL	0	NULL	controls 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Midluteal progesterone ( P ) and estradiol ( E2 ) were determined in 91 clip patients ; 21 normal worn and 27 tubal ligation cases served as controls .
	manualset3
108739	1	402949	5	NULL	NULL	0	NULL	Midwifery education	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Midwifery education is undergoing a curriculum revolution that is reflective of current trends in other fields .
	manualset3
108740	2	402949	5	NULL	NULL	0	NULL	curriculum revolution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Midwifery education is undergoing a curriculum revolution that is reflective of current trends in other fields .
	manualset3
108741	3	402949	5	NULL	NULL	0	NULL	current trends	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Midwifery education is undergoing a curriculum revolution that is reflective of current trends in other fields .
	manualset3
108742	4	402949	5	NULL	NULL	0	NULL	other fields	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Midwifery education is undergoing a curriculum revolution that is reflective of current trends in other fields .
	manualset3
108743	1	402950	5	NULL	NULL	0	NULL	Mifepristone 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Mifepristone for the prevention of breakthrough bleeding in new starters of depo-medroxyprogesterone acetate .
	manualset3
108744	2	402950	5	NULL	NULL	0	NULL	prevention 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Mifepristone for the prevention of breakthrough bleeding in new starters of depo-medroxyprogesterone acetate .
	manualset3
108745	3	402950	5	NULL	NULL	0	NULL	breakthrough bleeding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mifepristone for the prevention of breakthrough bleeding in new starters of depo-medroxyprogesterone acetate .
	manualset3
108746	4	402950	5	NULL	NULL	0	NULL	new starters	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mifepristone for the prevention of breakthrough bleeding in new starters of depo-medroxyprogesterone acetate .
	manualset3
108747	5	402950	5	NULL	NULL	0	NULL	depo-medroxyprogesterone acetate	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Mifepristone for the prevention of breakthrough bleeding in new starters of depo-medroxyprogesterone acetate .
	manualset3
108748	1	402951	5	NULL	NULL	0	NULL	case 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of Henoch-Schnlein purpura ( HSP ) with renal lesions is presented .
	manualset3
108749	2	402951	5	NULL	NULL	0	NULL	Henoch-Schnlein purpura ( HSP )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of Henoch-Schnlein purpura ( HSP ) with renal lesions is presented .
	manualset3
108750	3	402951	5	NULL	NULL	0	NULL	renal lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of Henoch-Schnlein purpura ( HSP ) with renal lesions is presented .
	manualset3
108751	1	402952	5	NULL	NULL	0	NULL	Migration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Migration into ethanol was dependent on both mass and thickness .
	manualset3
108752	2	402952	5	NULL	NULL	0	NULL	ethanol 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Migration into ethanol was dependent on both mass and thickness .
	manualset3
108753	3	402952	5	NULL	NULL	0	NULL	mass 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Migration into ethanol was dependent on both mass and thickness .
	manualset3
108754	4	402952	5	NULL	NULL	0	NULL	thickness 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Migration into ethanol was dependent on both mass and thickness .
	manualset3
108755	1	402953	5	NULL	NULL	0	NULL	Mild angular acceleration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Mild angular acceleration was imparted to the skull of a human volunteer inside an MR scanner , using a custom MR-compatible device to constrain motion .
	manualset3
108756	2	402953	5	NULL	NULL	0	NULL	skull 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mild angular acceleration was imparted to the skull of a human volunteer inside an MR scanner , using a custom MR-compatible device to constrain motion .
	manualset3
108757	3	402953	5	NULL	NULL	0	NULL	human volunteer	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Mild angular acceleration was imparted to the skull of a human volunteer inside an MR scanner , using a custom MR-compatible device to constrain motion .
	manualset3
108758	4	402953	5	NULL	NULL	0	NULL	MR scanner	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Mild angular acceleration was imparted to the skull of a human volunteer inside an MR scanner , using a custom MR-compatible device to constrain motion .
	manualset3
108759	5	402953	5	NULL	NULL	0	NULL	custom MR-compatible device	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Mild angular acceleration was imparted to the skull of a human volunteer inside an MR scanner , using a custom MR-compatible device to constrain motion .
	manualset3
108760	6	402953	5	NULL	NULL	0	NULL	motion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mild angular acceleration was imparted to the skull of a human volunteer inside an MR scanner , using a custom MR-compatible device to constrain motion .
	manualset3
108761	1	402954	5	NULL	NULL	0	NULL	Mild eosinophilia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mild eosinophilia was seen in two women and this reverted to normal on its own .
	manualset3
108762	2	402954	5	NULL	NULL	0	NULL	two women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mild eosinophilia was seen in two women and this reverted to normal on its own .
	manualset3
108763	1	402955	5	NULL	NULL	NULL	NULL	Mild hypothermia	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mild hypothermia is a technique that may soon be commonly employed alone or in conjunction with other methods of neuroprotection .
	manualset3
108764	2	402955	5	NULL	NULL	NULL	NULL	technique 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mild hypothermia is a technique that may soon be commonly employed alone or in conjunction with other methods of neuroprotection .
	manualset3
108765	3	402955	5	NULL	NULL	0	NULL	conjunction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mild hypothermia is a technique that may soon be commonly employed alone or in conjunction with other methods of neuroprotection .
	manualset3
108766	4	402955	5	NULL	NULL	0	NULL	methods 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mild hypothermia is a technique that may soon be commonly employed alone or in conjunction with other methods of neuroprotection .
	manualset3
108767	5	402955	5	NULL	NULL	0	NULL	neuroprotection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mild hypothermia is a technique that may soon be commonly employed alone or in conjunction with other methods of neuroprotection .
	manualset3
108768	1	402956	5	NULL	NULL	0	NULL	Milk-like fluid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Milk-like fluid in a mammary adenocarcinoma : biochemical characterization .
	manualset3
108769	2	402956	5	NULL	NULL	0	NULL	mammary adenocarcinoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Milk-like fluid in a mammary adenocarcinoma : biochemical characterization .
	manualset3
108770	3	402956	5	NULL	NULL	0	NULL	biochemical characterization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Milk-like fluid in a mammary adenocarcinoma : biochemical characterization .
	manualset3
108771	1	402957	5	NULL	NULL	0	NULL	Milk 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Milk contained more selenium from apparently absorbed SeMet than from selenite .
	manualset3
108772	2	402957	5	NULL	NULL	0	NULL	selenium 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Milk contained more selenium from apparently absorbed SeMet than from selenite .
	manualset3
108773	3	402957	5	NULL	NULL	0	NULL	SeMet	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Milk contained more selenium from apparently absorbed SeMet than from selenite .
	manualset3
108774	4	402957	5	NULL	NULL	0	NULL	selenite 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Milk contained more selenium from apparently absorbed SeMet than from selenite .
	manualset3
108775	1	402958	5	NULL	NULL	0	NULL	Milk stasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Milk stasis , blocked ducts , inflammatory or infectious mastitis , and breast abscess represent the spectrum of maternal hyperlactation syndrome .
	manualset3
108776	2	402958	5	NULL	NULL	0	NULL	blocked ducts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Milk stasis , blocked ducts , inflammatory or infectious mastitis , and breast abscess represent the spectrum of maternal hyperlactation syndrome .
	manualset3
108777	3	402958	5	NULL	NULL	0	NULL	inflammatory or infectious mastitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Milk stasis , blocked ducts , inflammatory or infectious mastitis , and breast abscess represent the spectrum of maternal hyperlactation syndrome .
	manualset3
108778	4	402958	5	NULL	NULL	0	NULL	breast abscess	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Milk stasis , blocked ducts , inflammatory or infectious mastitis , and breast abscess represent the spectrum of maternal hyperlactation syndrome .
	manualset3
108779	5	402958	5	NULL	NULL	0	NULL	spectrum	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Milk stasis , blocked ducts , inflammatory or infectious mastitis , and breast abscess represent the spectrum of maternal hyperlactation syndrome .
	manualset3
108780	6	402958	5	NULL	NULL	0	NULL	maternal hyperlactation syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Milk stasis , blocked ducts , inflammatory or infectious mastitis , and breast abscess represent the spectrum of maternal hyperlactation syndrome .
	manualset3
108781	1	402959	5	NULL	NULL	0	NULL	Milk production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Milk production and reproductive performance in dairy cows given bovine respiratory syncytial virus vaccine prior to parturition .
	manualset3
108782	2	402959	5	NULL	NULL	0	NULL	reproductive performance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Milk production and reproductive performance in dairy cows given bovine respiratory syncytial virus vaccine prior to parturition .
	manualset3
108783	3	402959	5	NULL	NULL	0	NULL	dairy cows	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Milk production and reproductive performance in dairy cows given bovine respiratory syncytial virus vaccine prior to parturition .
	manualset3
108784	4	402959	5	NULL	NULL	0	NULL	bovine respiratory syncytial virus vaccine	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Milk production and reproductive performance in dairy cows given bovine respiratory syncytial virus vaccine prior to parturition .
	manualset3
108785	5	402959	5	NULL	NULL	0	NULL	parturition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Milk production and reproductive performance in dairy cows given bovine respiratory syncytial virus vaccine prior to parturition .
	manualset3
108786	1	402960	5	NULL	NULL	0	NULL	case 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of Pneumocystis carinii pneumonia was induced through immunosuppression following thoracic duct ligation .
	manualset3
108787	2	402960	5	NULL	NULL	0	NULL	Pneumocystis carinii pneumonia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of Pneumocystis carinii pneumonia was induced through immunosuppression following thoracic duct ligation .
	manualset3
108788	3	402960	5	NULL	NULL	0	NULL	immunosuppression 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of Pneumocystis carinii pneumonia was induced through immunosuppression following thoracic duct ligation .
	manualset3
108789	4	402960	5	NULL	NULL	0	NULL	thoracic duct ligation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of Pneumocystis carinii pneumonia was induced through immunosuppression following thoracic duct ligation .
	manualset3
108790	1	402961	5	NULL	NULL	0	NULL	Milli-calpain	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Milli-calpain from sea bass ( Dicentrarchus labrax ) white muscle : purification , characterization of its activity and activation in vitro .
	manualset3
108791	2	402961	5	NULL	NULL	0	NULL	sea bass ( Dicentrarchus labrax ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Milli-calpain from sea bass ( Dicentrarchus labrax ) white muscle : purification , characterization of its activity and activation in vitro .
	manualset3
108792	3	402961	5	NULL	NULL	0	NULL	white muscle	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Milli-calpain from sea bass ( Dicentrarchus labrax ) white muscle : purification , characterization of its activity and activation in vitro .
	manualset3
108794	4	402961	5	NULL	NULL	0	NULL	purification 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Milli-calpain from sea bass ( Dicentrarchus labrax ) white muscle : purification , characterization of its activity and activation in vitro .
	manualset3
108795	5	402961	5	NULL	NULL	0	NULL	characterization 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Milli-calpain from sea bass ( Dicentrarchus labrax ) white muscle : purification , characterization of its activity and activation in vitro .
	manualset3
108796	6	402961	5	NULL	NULL	0	NULL	activity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Milli-calpain from sea bass ( Dicentrarchus labrax ) white muscle : purification , characterization of its activity and activation in vitro .
	manualset3
108797	7	402961	5	NULL	NULL	0	NULL	activation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Milli-calpain from sea bass ( Dicentrarchus labrax ) white muscle : purification , characterization of its activity and activation in vitro .
	manualset3
108798	1	402962	5	NULL	NULL	0	NULL	Millions 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Millions of healthy women use combined oral contraceptives ( o.c. ) for decades .
	manualset3
108799	2	402962	5	NULL	NULL	0	NULL	healthy women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Millions of healthy women use combined oral contraceptives ( o.c. ) for decades .
	manualset3
108800	3	402962	5	NULL	NULL	0	NULL	combined oral contraceptives ( o.c. ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Millions of healthy women use combined oral contraceptives ( o.c. ) for decades .
	manualset3
108801	4	402962	5	NULL	NULL	0	NULL	decades	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Millions of healthy women use combined oral contraceptives ( o.c. ) for decades .
	manualset3
108802	1	402963	5	NULL	NULL	0	NULL	Mini-CG	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Mini-CG contains a d ( CG ) 7 insert which assumes a left-handed Z-DNA conformation in negative supercoiled topoisomers with a negative linking number difference - delta Lk greater than or equal to 2 .
	manualset3
108803	2	402963	5	NULL	NULL	0	NULL	d ( CG ) 7 insert	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Mini-CG contains a d ( CG ) 7 insert which assumes a left-handed Z-DNA conformation in negative supercoiled topoisomers with a negative linking number difference - delta Lk greater than or equal to 2 .
	manualset3
108804	3	402963	5	NULL	NULL	0	NULL	left-handed Z-DNA conformation	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Mini-CG contains a d ( CG ) 7 insert which assumes a left-handed Z-DNA conformation in negative supercoiled topoisomers with a negative linking number difference - delta Lk greater than or equal to 2 .
	manualset3
108805	4	402963	5	NULL	NULL	0	NULL	negative supercoiled topoisomers	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mini-CG contains a d ( CG ) 7 insert which assumes a left-handed Z-DNA conformation in negative supercoiled topoisomers with a negative linking number difference - delta Lk greater than or equal to 2 .
	manualset3
108806	5	402963	5	NULL	NULL	0	NULL	negative linking number difference	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mini-CG contains a d ( CG ) 7 insert which assumes a left-handed Z-DNA conformation in negative supercoiled topoisomers with a negative linking number difference - delta Lk greater than or equal to 2 .
	manualset3
108807	6	402963	5	NULL	NULL	0	NULL	delta Lk	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mini-CG contains a d ( CG ) 7 insert which assumes a left-handed Z-DNA conformation in negative supercoiled topoisomers with a negative linking number difference - delta Lk greater than or equal to 2 .
	manualset3
108808	7	402963	5	NULL	NULL	0	NULL	2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mini-CG contains a d ( CG ) 7 insert which assumes a left-handed Z-DNA conformation in negative supercoiled topoisomers with a negative linking number difference - delta Lk greater than or equal to 2 .
	manualset3
108809	1	402964	5	NULL	NULL	0	NULL	Health Assessment Questionnaire	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Minimally important difference of Health Assessment Questionnaire in psoriatic arthritis : relating thresholds of improvement in functional ability to patient-rated importance and satisfaction .
	manualset3
108810	2	402964	5	NULL	NULL	0	NULL	psoriatic arthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Minimally important difference of Health Assessment Questionnaire in psoriatic arthritis : relating thresholds of improvement in functional ability to patient-rated importance and satisfaction .
	manualset3
108811	3	402964	5	NULL	NULL	NULL	NULL	thresholds	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Minimally important difference of Health Assessment Questionnaire in psoriatic arthritis : relating thresholds of improvement in functional ability to patient-rated importance and satisfaction .
	manualset3
108812	4	402964	5	NULL	NULL	0	NULL	improvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Minimally important difference of Health Assessment Questionnaire in psoriatic arthritis : relating thresholds of improvement in functional ability to patient-rated importance and satisfaction .
	manualset3
108813	5	402964	5	NULL	NULL	0	NULL	functional ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Minimally important difference of Health Assessment Questionnaire in psoriatic arthritis : relating thresholds of improvement in functional ability to patient-rated importance and satisfaction .
	manualset3
108814	6	402964	5	NULL	NULL	0	NULL	patient-rated importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Minimally important difference of Health Assessment Questionnaire in psoriatic arthritis : relating thresholds of improvement in functional ability to patient-rated importance and satisfaction .
	manualset3
108815	7	402964	5	NULL	NULL	0	NULL	satisfaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Minimally important difference of Health Assessment Questionnaire in psoriatic arthritis : relating thresholds of improvement in functional ability to patient-rated importance and satisfaction .
	manualset3
108816	1	402965	5	NULL	NULL	0	NULL	Minimally invasive biopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Minimally invasive biopsy can permit accurate diagnosis and prompt intervention in a cost-effective manner , particularly in countries with limited resources , where patients often present with advanced-stage breast cancer .
	manualset3
108817	2	402965	5	NULL	NULL	0	NULL	accurate diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Minimally invasive biopsy can permit accurate diagnosis and prompt intervention in a cost-effective manner , particularly in countries with limited resources , where patients often present with advanced-stage breast cancer .
	manualset3
108818	3	402965	5	NULL	NULL	0	NULL	prompt intervention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Minimally invasive biopsy can permit accurate diagnosis and prompt intervention in a cost-effective manner , particularly in countries with limited resources , where patients often present with advanced-stage breast cancer .
	manualset3
108819	4	402965	5	NULL	NULL	0	NULL	cost-effective manner	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Minimally invasive biopsy can permit accurate diagnosis and prompt intervention in a cost-effective manner , particularly in countries with limited resources , where patients often present with advanced-stage breast cancer .
	manualset3
108820	5	402965	5	NULL	NULL	0	NULL	countries	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Minimally invasive biopsy can permit accurate diagnosis and prompt intervention in a cost-effective manner , particularly in countries with limited resources , where patients often present with advanced-stage breast cancer .
	manualset3
108821	6	402965	5	NULL	NULL	0	NULL	limited resources	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Minimally invasive biopsy can permit accurate diagnosis and prompt intervention in a cost-effective manner , particularly in countries with limited resources , where patients often present with advanced-stage breast cancer .
	manualset3
108822	7	402965	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Minimally invasive biopsy can permit accurate diagnosis and prompt intervention in a cost-effective manner , particularly in countries with limited resources , where patients often present with advanced-stage breast cancer .
	manualset3
108823	8	402965	5	NULL	NULL	0	NULL	advanced-stage breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Minimally invasive biopsy can permit accurate diagnosis and prompt intervention in a cost-effective manner , particularly in countries with limited resources , where patients often present with advanced-stage breast cancer .
	manualset3
108824	1	402966	5	NULL	NULL	0	NULL	skin exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Minimizing skin exposure , providing adequate bed linen for the transfer to theater and educating patients about the importance of keeping warm perioperatively are all extremely important .
	manualset3
108825	2	402966	5	NULL	NULL	0	NULL	adequate bed linen	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Minimizing skin exposure , providing adequate bed linen for the transfer to theater and educating patients about the importance of keeping warm perioperatively are all extremely important .
	manualset3
108826	3	402966	5	NULL	NULL	0	NULL	theater	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Minimizing skin exposure , providing adequate bed linen for the transfer to theater and educating patients about the importance of keeping warm perioperatively are all extremely important .
	manualset3
108827	4	402966	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Minimizing skin exposure , providing adequate bed linen for the transfer to theater and educating patients about the importance of keeping warm perioperatively are all extremely important .
	manualset3
108828	5	402966	5	NULL	NULL	0	NULL	importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Minimizing skin exposure , providing adequate bed linen for the transfer to theater and educating patients about the importance of keeping warm perioperatively are all extremely important .
	manualset3
108829	1	402967	5	NULL	NULL	0	NULL	iatrogenic injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Minimizing this iatrogenic injury can help achieve the goals of the minimally invasive approach : decreased postoperative pain , decreased blood loss , and faster rehabilitation .
	manualset3
108830	2	402967	5	NULL	NULL	0	NULL	goals	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Minimizing this iatrogenic injury can help achieve the goals of the minimally invasive approach : decreased postoperative pain , decreased blood loss , and faster rehabilitation .
	manualset3
108831	3	402967	5	NULL	NULL	0	NULL	minimally invasive approach	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Minimizing this iatrogenic injury can help achieve the goals of the minimally invasive approach : decreased postoperative pain , decreased blood loss , and faster rehabilitation .
	manualset3
108832	4	402967	5	NULL	NULL	0	NULL	postoperative pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Minimizing this iatrogenic injury can help achieve the goals of the minimally invasive approach : decreased postoperative pain , decreased blood loss , and faster rehabilitation .
	manualset3
108833	5	402967	5	NULL	NULL	0	NULL	blood loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Minimizing this iatrogenic injury can help achieve the goals of the minimally invasive approach : decreased postoperative pain , decreased blood loss , and faster rehabilitation .
	manualset3
108834	6	402967	5	NULL	NULL	0	NULL	rehabilitation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Minimizing this iatrogenic injury can help achieve the goals of the minimally invasive approach : decreased postoperative pain , decreased blood loss , and faster rehabilitation .
	manualset3
108835	1	402968	5	NULL	NULL	NULL	NULL	Minor fish mortality	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Minor fish mortality occurred only in shallow water exposed to direct spray .
	manualset3
108836	2	402968	5	NULL	NULL	0	NULL	shallow water	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Minor fish mortality occurred only in shallow water exposed to direct spray .
	manualset3
108837	3	402968	5	NULL	NULL	0	NULL	direct spray	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Minor fish mortality occurred only in shallow water exposed to direct spray .
	manualset3
108838	1	402969	5	NULL	NULL	0	NULL	case	person												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of Sick Sinus Syndrome probably secondary to cardiac metastasis in a patient affected by metastatic breast cancer is described .
	manualset3
108839	2	402969	5	NULL	NULL	NULL	NULL	Sick Sinus Syndrome	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A case of Sick Sinus Syndrome probably secondary to cardiac metastasis in a patient affected by metastatic breast cancer is described .
	manualset3
108840	3	402969	5	NULL	NULL	0	NULL	cardiac metastasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of Sick Sinus Syndrome probably secondary to cardiac metastasis in a patient affected by metastatic breast cancer is described .
	manualset3
108841	4	402969	5	NULL	NULL	0	NULL	patient	person												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of Sick Sinus Syndrome probably secondary to cardiac metastasis in a patient affected by metastatic breast cancer is described .
	manualset3
108842	5	402969	5	NULL	NULL	0	NULL	metastatic breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of Sick Sinus Syndrome probably secondary to cardiac metastasis in a patient affected by metastatic breast cancer is described .
	manualset3
108843	1	402970	5	NULL	NULL	0	NULL	Minor side effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Minor side effects such as fever and pain were observed .
	manualset3
108844	2	402970	5	NULL	NULL	0	NULL	fever	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Minor side effects such as fever and pain were observed .
	manualset3
108845	3	402970	5	NULL	NULL	0	NULL	pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Minor side effects such as fever and pain were observed .
	manualset3
108846	1	402971	5	NULL	NULL	0	NULL	Minority women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Minority women are particularly vulnerable because of environmental stress .
	manualset3
108847	2	402971	5	NULL	NULL	0	NULL	environmental stress	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Minority women are particularly vulnerable because of environmental stress .
	manualset3
108848	1	402972	5	NULL	NULL	0	NULL	behavior	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Minute-to-minute behavior of the bowel , whether it is normal or disordered , is determined by integrative functions of the enteric nervous system ( ENS ) .
	manualset3
108849	2	402972	5	NULL	NULL	0	NULL	bowel	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Minute-to-minute behavior of the bowel , whether it is normal or disordered , is determined by integrative functions of the enteric nervous system ( ENS ) .
	manualset3
108850	3	402972	5	NULL	NULL	0	NULL	integrative functions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Minute-to-minute behavior of the bowel , whether it is normal or disordered , is determined by integrative functions of the enteric nervous system ( ENS ) .
	manualset3
108851	4	402972	5	NULL	NULL	0	NULL	enteric nervous system ( ENS )	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Minute-to-minute behavior of the bowel , whether it is normal or disordered , is determined by integrative functions of the enteric nervous system ( ENS ) .
	manualset3
108852	1	402973	5	NULL	NULL	0	NULL	Misperceptions	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Misperceptions of patients vs providers regarding medication-related communication issues .
	manualset3
108853	2	402973	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Misperceptions of patients vs providers regarding medication-related communication issues .
	manualset3
108854	3	402973	5	NULL	NULL	0	NULL	providers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Misperceptions of patients vs providers regarding medication-related communication issues .
	manualset3
108855	4	402973	5	NULL	NULL	0	NULL	medication-related communication issues	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Misperceptions of patients vs providers regarding medication-related communication issues .
	manualset3
108856	1	402974	5	NULL	NULL	0	NULL	Mite diversity	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mite diversity was the highest in the state Par and on palms surrounded by seasonal forests and Amazonian rain-forests .
	manualset3
108857	2	402974	5	NULL	NULL	0	NULL	state Par	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Mite diversity was the highest in the state Par and on palms surrounded by seasonal forests and Amazonian rain-forests .
	manualset3
108858	3	402974	5	NULL	NULL	0	NULL	palms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mite diversity was the highest in the state Par and on palms surrounded by seasonal forests and Amazonian rain-forests .
	manualset3
108859	4	402974	5	NULL	NULL	0	NULL	seasonal forests	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Mite diversity was the highest in the state Par and on palms surrounded by seasonal forests and Amazonian rain-forests .
	manualset3
108860	5	402974	5	NULL	NULL	0	NULL	Amazonian rain-forests	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Mite diversity was the highest in the state Par and on palms surrounded by seasonal forests and Amazonian rain-forests .
	manualset3
108861	1	402975	5	NULL	NULL	0	NULL	Mitochondrial ATP synthase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial ATP synthase : dramatic Mg2 + - induced alterations in the structure and function of the F1-ATPase moiety .
	manualset3
108862	2	402975	5	NULL	NULL	0	NULL	Mg2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial ATP synthase : dramatic Mg2 + - induced alterations in the structure and function of the F1-ATPase moiety .
	manualset3
108863	3	402975	5	NULL	NULL	0	NULL	alterations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial ATP synthase : dramatic Mg2 + - induced alterations in the structure and function of the F1-ATPase moiety .
	manualset3
108864	4	402975	5	NULL	NULL	0	NULL	structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial ATP synthase : dramatic Mg2 + - induced alterations in the structure and function of the F1-ATPase moiety .
	manualset3
108865	5	402975	5	NULL	NULL	0	NULL	function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial ATP synthase : dramatic Mg2 + - induced alterations in the structure and function of the F1-ATPase moiety .
	manualset3
108866	6	402975	5	NULL	NULL	0	NULL	F1-ATPase moiety	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial ATP synthase : dramatic Mg2 + - induced alterations in the structure and function of the F1-ATPase moiety .
	manualset3
108867	1	402976	5	NULL	NULL	0	NULL	Mitochondrial ATPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial ATPase from rat liver mitochondria contains multiple nucleotide binding sites .
	manualset3
108868	2	402976	5	NULL	NULL	0	NULL	rat liver mitochondria	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial ATPase from rat liver mitochondria contains multiple nucleotide binding sites .
	manualset3
108869	3	402976	5	NULL	NULL	0	NULL	multiple nucleotide binding sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial ATPase from rat liver mitochondria contains multiple nucleotide binding sites .
	manualset3
108870	1	402977	5	NULL	NULL	0	NULL	Mitochondrial calcium granules	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial calcium granules were found in less than 3 % of the cells , and in these the cytoplasmic K/Na ratio was reduced , indicating that they were damaged .
	manualset3
108871	2	402977	5	NULL	NULL	0	NULL	3 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial calcium granules were found in less than 3 % of the cells , and in these the cytoplasmic K/Na ratio was reduced , indicating that they were damaged .
	manualset3
108872	3	402977	5	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial calcium granules were found in less than 3 % of the cells , and in these the cytoplasmic K/Na ratio was reduced , indicating that they were damaged .
	manualset3
108873	4	402977	5	NULL	NULL	0	NULL	cytoplasmic K/Na ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial calcium granules were found in less than 3 % of the cells , and in these the cytoplasmic K/Na ratio was reduced , indicating that they were damaged .
	manualset3
108874	1	402978	5	NULL	NULL	0	NULL	Mitochondrial carriers	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial carriers link biochemical pathways in the cytosol and mitochondrial matrix by transporting substrates across the inner mitochondrial membrane .
	manualset3
108875	2	402978	5	NULL	NULL	0	NULL	biochemical pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial carriers link biochemical pathways in the cytosol and mitochondrial matrix by transporting substrates across the inner mitochondrial membrane .
	manualset3
108876	3	402978	5	NULL	NULL	0	NULL	cytosol	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial carriers link biochemical pathways in the cytosol and mitochondrial matrix by transporting substrates across the inner mitochondrial membrane .
	manualset3
108877	4	402978	5	NULL	NULL	0	NULL	mitochondrial matrix	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial carriers link biochemical pathways in the cytosol and mitochondrial matrix by transporting substrates across the inner mitochondrial membrane .
	manualset3
108878	5	402978	5	NULL	NULL	0	NULL	transporting substrates	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial carriers link biochemical pathways in the cytosol and mitochondrial matrix by transporting substrates across the inner mitochondrial membrane .
	manualset3
108879	6	402978	5	NULL	NULL	0	NULL	inner mitochondrial membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial carriers link biochemical pathways in the cytosol and mitochondrial matrix by transporting substrates across the inner mitochondrial membrane .
	manualset3
108880	1	402979	5	NULL	NULL	0	NULL	Mitochondrial cytochrome c oxidase subunit 1 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial cytochrome c oxidase subunit 1 gene and nuclear rDNA regions of Enterobius vermicularis parasitic in captive chimpanzees with special reference to its relationship with pinworms in humans .
	manualset3
108881	2	402979	5	NULL	NULL	0	NULL	nuclear rDNA regions	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial cytochrome c oxidase subunit 1 gene and nuclear rDNA regions of Enterobius vermicularis parasitic in captive chimpanzees with special reference to its relationship with pinworms in humans .
	manualset3
108882	3	402979	5	NULL	NULL	0	NULL	Enterobius vermicularis parasitic	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial cytochrome c oxidase subunit 1 gene and nuclear rDNA regions of Enterobius vermicularis parasitic in captive chimpanzees with special reference to its relationship with pinworms in humans .
	manualset3
108883	4	402979	5	NULL	NULL	0	NULL	captive chimpanzees	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial cytochrome c oxidase subunit 1 gene and nuclear rDNA regions of Enterobius vermicularis parasitic in captive chimpanzees with special reference to its relationship with pinworms in humans .
	manualset3
108884	5	402979	5	NULL	NULL	0	NULL	special reference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial cytochrome c oxidase subunit 1 gene and nuclear rDNA regions of Enterobius vermicularis parasitic in captive chimpanzees with special reference to its relationship with pinworms in humans .
	manualset3
108885	6	402979	5	NULL	NULL	0	NULL	relationship	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial cytochrome c oxidase subunit 1 gene and nuclear rDNA regions of Enterobius vermicularis parasitic in captive chimpanzees with special reference to its relationship with pinworms in humans .
	manualset3
108886	7	402979	5	NULL	NULL	0	NULL	pinworms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial cytochrome c oxidase subunit 1 gene and nuclear rDNA regions of Enterobius vermicularis parasitic in captive chimpanzees with special reference to its relationship with pinworms in humans .
	manualset3
108887	8	402979	5	NULL	NULL	0	NULL	humans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial cytochrome c oxidase subunit 1 gene and nuclear rDNA regions of Enterobius vermicularis parasitic in captive chimpanzees with special reference to its relationship with pinworms in humans .
	manualset3
108888	1	402980	5	NULL	NULL	NULL	NULL	Mitochondrial damage	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mitochondrial damage is one of the prominent features of cell injury during oxidative stress and altered mitochondrial lipids may contribute to this damage .
	manualset3
108889	2	402980	5	NULL	NULL	0	NULL	prominent features	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial damage is one of the prominent features of cell injury during oxidative stress and altered mitochondrial lipids may contribute to this damage .
	manualset3
108890	3	402980	5	NULL	NULL	0	NULL	cell injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial damage is one of the prominent features of cell injury during oxidative stress and altered mitochondrial lipids may contribute to this damage .
	manualset3
108891	4	402980	5	NULL	NULL	0	NULL	oxidative stress	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial damage is one of the prominent features of cell injury during oxidative stress and altered mitochondrial lipids may contribute to this damage .
	manualset3
108892	5	402980	5	NULL	NULL	0	NULL	altered mitochondrial lipids	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial damage is one of the prominent features of cell injury during oxidative stress and altered mitochondrial lipids may contribute to this damage .
	manualset3
108893	6	402980	5	NULL	NULL	0	NULL	damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitochondrial damage is one of the prominent features of cell injury during oxidative stress and altered mitochondrial lipids may contribute to this damage .
	manualset3
108894	1	402981	5	NULL	NULL	0	NULL	Mitogen effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitogen effects on lipid metabolism during lymphocyte activation .
	manualset3
108895	2	402981	5	NULL	NULL	0	NULL	lipid metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitogen effects on lipid metabolism during lymphocyte activation .
	manualset3
108896	3	402981	5	NULL	NULL	0	NULL	lymphocyte activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitogen effects on lipid metabolism during lymphocyte activation .
	manualset3
108897	1	402982	5	NULL	NULL	0	NULL	Mitral annulus calcification ( MAC )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitral annulus calcification ( MAC ) is an independent predictor of coronary artery disease ( CAD ) .
	manualset3
108898	2	402982	5	NULL	NULL	0	NULL	independent predictor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitral annulus calcification ( MAC ) is an independent predictor of coronary artery disease ( CAD ) .
	manualset3
108899	3	402982	5	NULL	NULL	0	NULL	coronary artery disease ( CAD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitral annulus calcification ( MAC ) is an independent predictor of coronary artery disease ( CAD ) .
	manualset3
108900	1	402983	5	NULL	NULL	0	NULL	Mitral regurgitation	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitral regurgitation invariably accompanies the obstruction to outflow .
	manualset3
108901	2	402983	5	NULL	NULL	0	NULL	obstruction to outflow	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitral regurgitation invariably accompanies the obstruction to outflow .
	manualset3
108902	1	402984	5	NULL	NULL	0	NULL	Mitral valve ring abscess	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitral valve ring abscess and ventricular pseudoaneurysm are rare complications of infective endocarditis .
	manualset3
108903	2	402984	5	NULL	NULL	0	NULL	ventricular pseudoaneurysm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitral valve ring abscess and ventricular pseudoaneurysm are rare complications of infective endocarditis .
	manualset3
108904	3	402984	5	NULL	NULL	0	NULL	rare complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitral valve ring abscess and ventricular pseudoaneurysm are rare complications of infective endocarditis .
	manualset3
108905	4	402984	5	NULL	NULL	0	NULL	infective endocarditis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitral valve ring abscess and ventricular pseudoaneurysm are rare complications of infective endocarditis .
	manualset3
108906	1	402985	5	NULL	NULL	0	NULL	Mitral valve surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitral valve surgery with extensive calcification of the annulus .
	manualset3
108907	2	402985	5	NULL	NULL	0	NULL	extensive calcification	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitral valve surgery with extensive calcification of the annulus .
	manualset3
108908	3	402985	5	NULL	NULL	0	NULL	annulus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mitral valve surgery with extensive calcification of the annulus .
	manualset3
108909	1	402986	5	NULL	NULL	0	NULL	case	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of a patient with a fracture of the temporomandibular joint ( TMJ ) disk is reported .
	manualset3
108910	2	402986	5	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of a patient with a fracture of the temporomandibular joint ( TMJ ) disk is reported .
	manualset3
108911	3	402986	5	NULL	NULL	0	NULL	fracture	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of a patient with a fracture of the temporomandibular joint ( TMJ ) disk is reported .
	manualset3
108912	4	402986	5	NULL	NULL	0	NULL	temporomandibular joint ( TMJ ) disk	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of a patient with a fracture of the temporomandibular joint ( TMJ ) disk is reported .
	manualset3
108913	1	402987	5	NULL	NULL	0	NULL	Mixed bacillary population	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mixed bacillary population was found 2 times more frequently in patients with serious progressive forms of tuberculosis , which gives evidence to consider it as a prognostically unfavourable indicator .
	manualset3
108914	2	402987	5	NULL	NULL	0	NULL	2 times	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mixed bacillary population was found 2 times more frequently in patients with serious progressive forms of tuberculosis , which gives evidence to consider it as a prognostically unfavourable indicator .
	manualset3
108915	3	402987	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mixed bacillary population was found 2 times more frequently in patients with serious progressive forms of tuberculosis , which gives evidence to consider it as a prognostically unfavourable indicator .
	manualset3
108916	4	402987	5	NULL	NULL	0	NULL	serious progressive forms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mixed bacillary population was found 2 times more frequently in patients with serious progressive forms of tuberculosis , which gives evidence to consider it as a prognostically unfavourable indicator .
	manualset3
108917	5	402987	5	NULL	NULL	0	NULL	tuberculosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mixed bacillary population was found 2 times more frequently in patients with serious progressive forms of tuberculosis , which gives evidence to consider it as a prognostically unfavourable indicator .
	manualset3
108918	6	402987	5	NULL	NULL	0	NULL	evidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mixed bacillary population was found 2 times more frequently in patients with serious progressive forms of tuberculosis , which gives evidence to consider it as a prognostically unfavourable indicator .
	manualset3
108919	7	402987	5	NULL	NULL	NULL	NULL	unfavourable indicator	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mixed bacillary population was found 2 times more frequently in patients with serious progressive forms of tuberculosis , which gives evidence to consider it as a prognostically unfavourable indicator .
	manualset3
108920	1	402988	5	NULL	NULL	0	NULL	Mixed monolayers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mixed monolayers of poly ( methyl methacrylate ) ( PMMA ) , the main component of hard contact lenses , and dipalmitoyl phosphatidyl choline ( DPPC ) , a characteristic phospholipidic constituent of ocular tear films , were selected as an in vitro model in order to observe the behavior of contact lenses on the eye .
	manualset3
108921	2	402988	5	NULL	NULL	0	NULL	poly ( methyl methacrylate ) ( PMMA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mixed monolayers of poly ( methyl methacrylate ) ( PMMA ) , the main component of hard contact lenses , and dipalmitoyl phosphatidyl choline ( DPPC ) , a characteristic phospholipidic constituent of ocular tear films , were selected as an in vitro model in order to observe the behavior of contact lenses on the eye .
	manualset3
108922	3	402988	5	NULL	NULL	0	NULL	main component	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mixed monolayers of poly ( methyl methacrylate ) ( PMMA ) , the main component of hard contact lenses , and dipalmitoyl phosphatidyl choline ( DPPC ) , a characteristic phospholipidic constituent of ocular tear films , were selected as an in vitro model in order to observe the behavior of contact lenses on the eye .
	manualset3
108923	4	402988	5	NULL	NULL	0	NULL	hard contact lenses	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Mixed monolayers of poly ( methyl methacrylate ) ( PMMA ) , the main component of hard contact lenses , and dipalmitoyl phosphatidyl choline ( DPPC ) , a characteristic phospholipidic constituent of ocular tear films , were selected as an in vitro model in order to observe the behavior of contact lenses on the eye .
	manualset3
108924	5	402988	5	NULL	NULL	0	NULL	dipalmitoyl phosphatidyl choline ( DPPC )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mixed monolayers of poly ( methyl methacrylate ) ( PMMA ) , the main component of hard contact lenses , and dipalmitoyl phosphatidyl choline ( DPPC ) , a characteristic phospholipidic constituent of ocular tear films , were selected as an in vitro model in order to observe the behavior of contact lenses on the eye .
	manualset3
108925	6	402988	5	NULL	NULL	0	NULL	dipalmitoyl phosphatidyl choline ( DPPC )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Mixed monolayers of poly ( methyl methacrylate ) ( PMMA ) , the main component of hard contact lenses , and dipalmitoyl phosphatidyl choline ( DPPC ) , a characteristic phospholipidic constituent of ocular tear films , were selected as an in vitro model in order to observe the behavior of contact lenses on the eye .
	manualset3
108926	7	402988	5	NULL	NULL	0	NULL	phospholipidic constituent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mixed monolayers of poly ( methyl methacrylate ) ( PMMA ) , the main component of hard contact lenses , and dipalmitoyl phosphatidyl choline ( DPPC ) , a characteristic phospholipidic constituent of ocular tear films , were selected as an in vitro model in order to observe the behavior of contact lenses on the eye .
	manualset3
108927	8	402988	5	NULL	NULL	0	NULL	ocular tear films	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mixed monolayers of poly ( methyl methacrylate ) ( PMMA ) , the main component of hard contact lenses , and dipalmitoyl phosphatidyl choline ( DPPC ) , a characteristic phospholipidic constituent of ocular tear films , were selected as an in vitro model in order to observe the behavior of contact lenses on the eye .
	manualset3
108928	9	402988	5	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Mixed monolayers of poly ( methyl methacrylate ) ( PMMA ) , the main component of hard contact lenses , and dipalmitoyl phosphatidyl choline ( DPPC ) , a characteristic phospholipidic constituent of ocular tear films , were selected as an in vitro model in order to observe the behavior of contact lenses on the eye .
	manualset3
108930	11	402988	5	NULL	NULL	0	NULL	behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mixed monolayers of poly ( methyl methacrylate ) ( PMMA ) , the main component of hard contact lenses , and dipalmitoyl phosphatidyl choline ( DPPC ) , a characteristic phospholipidic constituent of ocular tear films , were selected as an in vitro model in order to observe the behavior of contact lenses on the eye .
	manualset3
108931	12	402988	5	NULL	NULL	0	NULL	contact lenses	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Mixed monolayers of poly ( methyl methacrylate ) ( PMMA ) , the main component of hard contact lenses , and dipalmitoyl phosphatidyl choline ( DPPC ) , a characteristic phospholipidic constituent of ocular tear films , were selected as an in vitro model in order to observe the behavior of contact lenses on the eye .
	manualset3
108932	13	402988	5	NULL	NULL	0	NULL	eye	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mixed monolayers of poly ( methyl methacrylate ) ( PMMA ) , the main component of hard contact lenses , and dipalmitoyl phosphatidyl choline ( DPPC ) , a characteristic phospholipidic constituent of ocular tear films , were selected as an in vitro model in order to observe the behavior of contact lenses on the eye .
	manualset3
108933	1	402989	5	NULL	NULL	0	NULL	repellents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mixing repellents and organophosphates on bed nets could be used to control insecticide-resistant malaria vectors if residual activity of the mixture is extended and safety is verified .
	manualset3
108934	2	402989	5	NULL	NULL	0	NULL	organophosphates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mixing repellents and organophosphates on bed nets could be used to control insecticide-resistant malaria vectors if residual activity of the mixture is extended and safety is verified .
	manualset3
108935	3	402989	5	NULL	NULL	0	NULL	bed nets	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	Mixing repellents and organophosphates on bed nets could be used to control insecticide-resistant malaria vectors if residual activity of the mixture is extended and safety is verified .
	manualset3
108936	4	402989	5	NULL	NULL	0	NULL	insecticide-resistant malaria vectors	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mixing repellents and organophosphates on bed nets could be used to control insecticide-resistant malaria vectors if residual activity of the mixture is extended and safety is verified .
	manualset3
108937	5	402989	5	NULL	NULL	0	NULL	residual activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mixing repellents and organophosphates on bed nets could be used to control insecticide-resistant malaria vectors if residual activity of the mixture is extended and safety is verified .
	manualset3
108938	6	402989	5	NULL	NULL	0	NULL	mixture	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mixing repellents and organophosphates on bed nets could be used to control insecticide-resistant malaria vectors if residual activity of the mixture is extended and safety is verified .
	manualset3
108939	7	402989	5	NULL	NULL	0	NULL	safety	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mixing repellents and organophosphates on bed nets could be used to control insecticide-resistant malaria vectors if residual activity of the mixture is extended and safety is verified .
	manualset3
108940	1	402990	5	NULL	NULL	0	NULL	Mllerian adenosarcoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mllerian adenosarcoma is a distinctive type of mixed Mllerian tumor of the female genital tract .
	manualset3
108941	2	402990	5	NULL	NULL	0	NULL	type	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mllerian adenosarcoma is a distinctive type of mixed Mllerian tumor of the female genital tract .
	manualset3
108942	3	402990	5	NULL	NULL	0	NULL	mixed Mllerian tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mllerian adenosarcoma is a distinctive type of mixed Mllerian tumor of the female genital tract .
	manualset3
108943	4	402990	5	NULL	NULL	0	NULL	female genital tract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mllerian adenosarcoma is a distinctive type of mixed Mllerian tumor of the female genital tract .
	manualset3
108944	1	402991	5	NULL	NULL	0	NULL	Mnemonic context effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mnemonic context effect in two cultures : attention to memory representations ?
	manualset3
108945	2	402991	5	NULL	NULL	0	NULL	two cultures	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Mnemonic context effect in two cultures : attention to memory representations ?
	manualset3
108946	3	402991	5	NULL	NULL	0	NULL	attention	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mnemonic context effect in two cultures : attention to memory representations ?
	manualset3
108947	4	402991	5	NULL	NULL	0	NULL	memory representations	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mnemonic context effect in two cultures : attention to memory representations ?
	manualset3
108948	1	402992	5	NULL	NULL	NULL	NULL	Mo	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mo repressed expression of both fusions whereas NH4 + and V repressed the anfA-lacZ fusion , but not the vnfA-lacZ fusion .
	manualset3
108949	2	402992	5	NULL	NULL	0	NULL	expression	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mo repressed expression of both fusions whereas NH4 + and V repressed the anfA-lacZ fusion , but not the vnfA-lacZ fusion .
	manualset3
108950	3	402992	5	NULL	NULL	0	NULL	fusions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mo repressed expression of both fusions whereas NH4 + and V repressed the anfA-lacZ fusion , but not the vnfA-lacZ fusion .
	manualset3
108951	4	402992	5	NULL	NULL	0	NULL	NH4 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Mo repressed expression of both fusions whereas NH4 + and V repressed the anfA-lacZ fusion , but not the vnfA-lacZ fusion .
	manualset3
108952	5	402992	5	NULL	NULL	0	NULL	vanadium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Mo repressed expression of both fusions whereas NH4 + and V repressed the anfA-lacZ fusion , but not the vnfA-lacZ fusion .
	manualset3
108953	6	402992	5	NULL	NULL	0	NULL	anfA-lacZ fusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mo repressed expression of both fusions whereas NH4 + and V repressed the anfA-lacZ fusion , but not the vnfA-lacZ fusion .
	manualset3
108954	7	402992	5	NULL	NULL	0	NULL	vnfA-lacZ fusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mo repressed expression of both fusions whereas NH4 + and V repressed the anfA-lacZ fusion , but not the vnfA-lacZ fusion .
	manualset3
108955	1	402993	5	NULL	NULL	0	NULL	action	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mode of action of LSD on serotonergic neurons .
	manualset3
108956	2	402993	5	NULL	NULL	0	NULL	LSD	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Mode of action of LSD on serotonergic neurons .
	manualset3
108957	3	402993	5	NULL	NULL	0	NULL	serotonergic neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mode of action of LSD on serotonergic neurons .
	manualset3
108958	1	402994	5	NULL	NULL	0	NULL	Model-building studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Model-building studies showed that when AdoP2Pxy is built into the open form of the enzyme , as described in X-ray studies , the pyridoxyl group of AdoP2Pxy can not reach Lys385 for Schiff-base formation .
	manualset3
108959	2	402994	5	NULL	NULL	0	NULL	AdoP2Pxy	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Model-building studies showed that when AdoP2Pxy is built into the open form of the enzyme , as described in X-ray studies , the pyridoxyl group of AdoP2Pxy can not reach Lys385 for Schiff-base formation .
	manualset3
108960	3	402994	5	NULL	NULL	0	NULL	open form of the enzyme	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Model-building studies showed that when AdoP2Pxy is built into the open form of the enzyme , as described in X-ray studies , the pyridoxyl group of AdoP2Pxy can not reach Lys385 for Schiff-base formation .
	manualset3
108961	4	402994	5	NULL	NULL	0	NULL	X-ray studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Model-building studies showed that when AdoP2Pxy is built into the open form of the enzyme , as described in X-ray studies , the pyridoxyl group of AdoP2Pxy can not reach Lys385 for Schiff-base formation .
	manualset3
108962	5	402994	5	NULL	NULL	NULL	NULL	pyridoxyl group	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Model-building studies showed that when AdoP2Pxy is built into the open form of the enzyme , as described in X-ray studies , the pyridoxyl group of AdoP2Pxy can not reach Lys385 for Schiff-base formation .
	manualset3
108963	6	402994	5	NULL	NULL	0	NULL	AdoP2Pxy	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Model-building studies showed that when AdoP2Pxy is built into the open form of the enzyme , as described in X-ray studies , the pyridoxyl group of AdoP2Pxy can not reach Lys385 for Schiff-base formation .
	manualset3
108964	7	402994	5	NULL	NULL	0	NULL	Lys385	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Model-building studies showed that when AdoP2Pxy is built into the open form of the enzyme , as described in X-ray studies , the pyridoxyl group of AdoP2Pxy can not reach Lys385 for Schiff-base formation .
	manualset3
108965	8	402994	5	NULL	NULL	0	NULL	Schiff-base formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Model-building studies showed that when AdoP2Pxy is built into the open form of the enzyme , as described in X-ray studies , the pyridoxyl group of AdoP2Pxy can not reach Lys385 for Schiff-base formation .
	manualset3
109089	1	402995	5	NULL	NULL	0	NULL	Model results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Model results indicate that non-uniform velocities significantly affect the diffusion coefficient and a range of diffusion coefficients should be considered when designing CSWs .
	manualset3
109090	2	402995	5	NULL	NULL	0	NULL	non-uniform velocities	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Model results indicate that non-uniform velocities significantly affect the diffusion coefficient and a range of diffusion coefficients should be considered when designing CSWs .
	manualset3
109091	3	402995	5	NULL	NULL	0	NULL	diffusion coefficient	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Model results indicate that non-uniform velocities significantly affect the diffusion coefficient and a range of diffusion coefficients should be considered when designing CSWs .
	manualset3
109092	4	402995	5	NULL	NULL	0	NULL	range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Model results indicate that non-uniform velocities significantly affect the diffusion coefficient and a range of diffusion coefficients should be considered when designing CSWs .
	manualset3
109093	5	402995	5	NULL	NULL	0	NULL	diffusion coefficients	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Model results indicate that non-uniform velocities significantly affect the diffusion coefficient and a range of diffusion coefficients should be considered when designing CSWs .
	manualset3
109094	6	402995	5	NULL	NULL	0	NULL	CSWs	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Model results indicate that non-uniform velocities significantly affect the diffusion coefficient and a range of diffusion coefficients should be considered when designing CSWs .
	manualset3
109095	1	402996	5	NULL	NULL	0	NULL	Model simulations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Model simulations of the oxidation of various organic species demonstrate the significant role organic radicals and oxidation byproducts can have on treatment performance .
	manualset3
109096	2	402996	5	NULL	NULL	0	NULL	oxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Model simulations of the oxidation of various organic species demonstrate the significant role organic radicals and oxidation byproducts can have on treatment performance .
	manualset3
109097	3	402996	5	NULL	NULL	NULL	NULL	organic species 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Model simulations of the oxidation of various organic species demonstrate the significant role organic radicals and oxidation byproducts can have on treatment performance .
	manualset3
109098	4	402996	5	NULL	NULL	0	NULL	significant role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Model simulations of the oxidation of various organic species demonstrate the significant role organic radicals and oxidation byproducts can have on treatment performance .
	manualset3
109099	5	402996	5	NULL	NULL	NULL	NULL	organic radicals	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Model simulations of the oxidation of various organic species demonstrate the significant role organic radicals and oxidation byproducts can have on treatment performance .
	manualset3
109100	6	402996	5	NULL	NULL	0	NULL	oxidation byproducts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Model simulations of the oxidation of various organic species demonstrate the significant role organic radicals and oxidation byproducts can have on treatment performance .
	manualset3
109101	7	402996	5	NULL	NULL	0	NULL	treatment performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Model simulations of the oxidation of various organic species demonstrate the significant role organic radicals and oxidation byproducts can have on treatment performance .
	manualset3
109102	1	402997	5	NULL	NULL	0	NULL	Modeling approaches	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Modeling approaches for the analysis of observer agreement .
	manualset3
109103	2	402997	5	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Modeling approaches for the analysis of observer agreement .
	manualset3
109104	3	402997	5	NULL	NULL	0	NULL	observer agreement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modeling approaches for the analysis of observer agreement .
	manualset3
109105	1	402998	5	NULL	NULL	NULL	NULL	Modeling climatic-change scenarios	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Modeling climatic-change scenarios is important to the development of conservation strategies .
	manualset3
109107	2	402998	5	NULL	NULL	NULL	NULL	development	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Modeling climatic-change scenarios is important to the development of conservation strategies .
	manualset3
109108	3	402998	5	NULL	NULL	NULL	NULL	conservation strategies	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Modeling climatic-change scenarios is important to the development of conservation strategies .
	manualset3
109109	1	402999	5	NULL	NULL	NULL	NULL	Modeling sharp wave-ripple complexes	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Modeling sharp wave-ripple complexes through a CA3-CA1 network model with chemical synapses .
	manualset3
109111	2	402999	5	NULL	NULL	NULL	NULL	CA3-CA1 network model	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Modeling sharp wave-ripple complexes through a CA3-CA1 network model with chemical synapses .
	manualset3
109112	3	402999	5	NULL	NULL	NULL	NULL	chemical synapses	AnatomicalPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Modeling sharp wave-ripple complexes through a CA3-CA1 network model with chemical synapses .
	manualset3
109113	1	403000	5	NULL	NULL	NULL	NULL	Modeling the effect	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Modeling the effect of reward amount on probability discounting .
	manualset3
109114	2	403000	5	NULL	NULL	0	NULL	reward amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Modeling the effect of reward amount on probability discounting .
	manualset3
109115	3	403000	5	NULL	NULL	0	NULL	probability discounting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modeling the effect of reward amount on probability discounting .
	manualset3
109116	1	403001	5	NULL	NULL	NULL	NULL	Modelling the growth	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Modelling the growth of soil-borne fungi in response to carbon and nitrogen .
	manualset3
109118	2	403001	5	NULL	NULL	NULL	NULL	soil-borne fungi	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Modelling the growth of soil-borne fungi in response to carbon and nitrogen .
	manualset3
109120	3	403001	5	NULL	NULL	NULL	NULL	carbon	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Modelling the growth of soil-borne fungi in response to carbon and nitrogen .
	manualset3
109121	4	403001	5	NULL	NULL	NULL	NULL	nitrogen	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Modelling the growth of soil-borne fungi in response to carbon and nitrogen .
	manualset3
109122	1	403002	5	NULL	NULL	0	NULL	case	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of cholesterosis bulbi with secondary glaucoma treated by vitrectomy and intravitreal bevacizumab .
	manualset3
109123	2	403002	5	NULL	NULL	0	NULL	cholesterosis bulbi	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of cholesterosis bulbi with secondary glaucoma treated by vitrectomy and intravitreal bevacizumab .
	manualset3
109124	3	403002	5	NULL	NULL	0	NULL	secondary glaucoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of cholesterosis bulbi with secondary glaucoma treated by vitrectomy and intravitreal bevacizumab .
	manualset3
109125	4	403002	5	NULL	NULL	0	NULL	vitrectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of cholesterosis bulbi with secondary glaucoma treated by vitrectomy and intravitreal bevacizumab .
	manualset3
109126	5	403002	5	NULL	NULL	0	NULL	intravitreal bevacizumab	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of cholesterosis bulbi with secondary glaucoma treated by vitrectomy and intravitreal bevacizumab .
	manualset3
109127	1	403003	5	NULL	NULL	0	NULL	Models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Models are presented that describe mechanisms for the transfer of mitochondrial DNA into the nucleus involving fragmentation of mitochondrial DNA through aging and/or oxidative damage , anomalous processing or escape of mitochondrial DNA and RNA fragments from autophagic vacuoles , and insertion of mitochondrial DNA sequences , in some instances after reverse transcription of mitochondrial RNA , into the nuclear genome .
	manualset3
109128	2	403003	5	NULL	NULL	0	NULL	mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Models are presented that describe mechanisms for the transfer of mitochondrial DNA into the nucleus involving fragmentation of mitochondrial DNA through aging and/or oxidative damage , anomalous processing or escape of mitochondrial DNA and RNA fragments from autophagic vacuoles , and insertion of mitochondrial DNA sequences , in some instances after reverse transcription of mitochondrial RNA , into the nuclear genome .
	manualset3
109129	3	403003	5	NULL	NULL	0	NULL	transfer	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Models are presented that describe mechanisms for the transfer of mitochondrial DNA into the nucleus involving fragmentation of mitochondrial DNA through aging and/or oxidative damage , anomalous processing or escape of mitochondrial DNA and RNA fragments from autophagic vacuoles , and insertion of mitochondrial DNA sequences , in some instances after reverse transcription of mitochondrial RNA , into the nuclear genome .
	manualset3
109130	4	403003	5	NULL	NULL	0	NULL	mitochondrial DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Models are presented that describe mechanisms for the transfer of mitochondrial DNA into the nucleus involving fragmentation of mitochondrial DNA through aging and/or oxidative damage , anomalous processing or escape of mitochondrial DNA and RNA fragments from autophagic vacuoles , and insertion of mitochondrial DNA sequences , in some instances after reverse transcription of mitochondrial RNA , into the nuclear genome .
	manualset3
109131	5	403003	5	NULL	NULL	0	NULL	nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Models are presented that describe mechanisms for the transfer of mitochondrial DNA into the nucleus involving fragmentation of mitochondrial DNA through aging and/or oxidative damage , anomalous processing or escape of mitochondrial DNA and RNA fragments from autophagic vacuoles , and insertion of mitochondrial DNA sequences , in some instances after reverse transcription of mitochondrial RNA , into the nuclear genome .
	manualset3
109132	6	403003	5	NULL	NULL	0	NULL	fragmentation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Models are presented that describe mechanisms for the transfer of mitochondrial DNA into the nucleus involving fragmentation of mitochondrial DNA through aging and/or oxidative damage , anomalous processing or escape of mitochondrial DNA and RNA fragments from autophagic vacuoles , and insertion of mitochondrial DNA sequences , in some instances after reverse transcription of mitochondrial RNA , into the nuclear genome .
	manualset3
109133	7	403003	5	NULL	NULL	0	NULL	mitochondrial DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Models are presented that describe mechanisms for the transfer of mitochondrial DNA into the nucleus involving fragmentation of mitochondrial DNA through aging and/or oxidative damage , anomalous processing or escape of mitochondrial DNA and RNA fragments from autophagic vacuoles , and insertion of mitochondrial DNA sequences , in some instances after reverse transcription of mitochondrial RNA , into the nuclear genome .
	manualset3
109134	8	403003	5	NULL	NULL	0	NULL	aging	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Models are presented that describe mechanisms for the transfer of mitochondrial DNA into the nucleus involving fragmentation of mitochondrial DNA through aging and/or oxidative damage , anomalous processing or escape of mitochondrial DNA and RNA fragments from autophagic vacuoles , and insertion of mitochondrial DNA sequences , in some instances after reverse transcription of mitochondrial RNA , into the nuclear genome .
	manualset3
109135	9	403003	5	NULL	NULL	0	NULL	oxidative damage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Models are presented that describe mechanisms for the transfer of mitochondrial DNA into the nucleus involving fragmentation of mitochondrial DNA through aging and/or oxidative damage , anomalous processing or escape of mitochondrial DNA and RNA fragments from autophagic vacuoles , and insertion of mitochondrial DNA sequences , in some instances after reverse transcription of mitochondrial RNA , into the nuclear genome .
	manualset3
109136	10	403003	5	NULL	NULL	0	NULL	anomalous processing	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Models are presented that describe mechanisms for the transfer of mitochondrial DNA into the nucleus involving fragmentation of mitochondrial DNA through aging and/or oxidative damage , anomalous processing or escape of mitochondrial DNA and RNA fragments from autophagic vacuoles , and insertion of mitochondrial DNA sequences , in some instances after reverse transcription of mitochondrial RNA , into the nuclear genome .
	manualset3
109137	11	403003	5	NULL	NULL	0	NULL	escape	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Models are presented that describe mechanisms for the transfer of mitochondrial DNA into the nucleus involving fragmentation of mitochondrial DNA through aging and/or oxidative damage , anomalous processing or escape of mitochondrial DNA and RNA fragments from autophagic vacuoles , and insertion of mitochondrial DNA sequences , in some instances after reverse transcription of mitochondrial RNA , into the nuclear genome .
	manualset3
109138	12	403003	5	NULL	NULL	0	NULL	mitochondrial DNA fragments	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Models are presented that describe mechanisms for the transfer of mitochondrial DNA into the nucleus involving fragmentation of mitochondrial DNA through aging and/or oxidative damage , anomalous processing or escape of mitochondrial DNA and RNA fragments from autophagic vacuoles , and insertion of mitochondrial DNA sequences , in some instances after reverse transcription of mitochondrial RNA , into the nuclear genome .
	manualset3
109139	13	403003	5	NULL	NULL	0	NULL	mitochondrial RNA fragments	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Models are presented that describe mechanisms for the transfer of mitochondrial DNA into the nucleus involving fragmentation of mitochondrial DNA through aging and/or oxidative damage , anomalous processing or escape of mitochondrial DNA and RNA fragments from autophagic vacuoles , and insertion of mitochondrial DNA sequences , in some instances after reverse transcription of mitochondrial RNA , into the nuclear genome .
	manualset3
109140	14	403003	5	NULL	NULL	0	NULL	autophagic vacuoles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Models are presented that describe mechanisms for the transfer of mitochondrial DNA into the nucleus involving fragmentation of mitochondrial DNA through aging and/or oxidative damage , anomalous processing or escape of mitochondrial DNA and RNA fragments from autophagic vacuoles , and insertion of mitochondrial DNA sequences , in some instances after reverse transcription of mitochondrial RNA , into the nuclear genome .
	manualset3
109141	15	403003	5	NULL	NULL	0	NULL	insertion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Models are presented that describe mechanisms for the transfer of mitochondrial DNA into the nucleus involving fragmentation of mitochondrial DNA through aging and/or oxidative damage , anomalous processing or escape of mitochondrial DNA and RNA fragments from autophagic vacuoles , and insertion of mitochondrial DNA sequences , in some instances after reverse transcription of mitochondrial RNA , into the nuclear genome .
	manualset3
109142	16	403003	5	NULL	NULL	0	NULL	mitochondrial DNA sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Models are presented that describe mechanisms for the transfer of mitochondrial DNA into the nucleus involving fragmentation of mitochondrial DNA through aging and/or oxidative damage , anomalous processing or escape of mitochondrial DNA and RNA fragments from autophagic vacuoles , and insertion of mitochondrial DNA sequences , in some instances after reverse transcription of mitochondrial RNA , into the nuclear genome .
	manualset3
109143	17	403003	5	NULL	NULL	0	NULL	instances	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Models are presented that describe mechanisms for the transfer of mitochondrial DNA into the nucleus involving fragmentation of mitochondrial DNA through aging and/or oxidative damage , anomalous processing or escape of mitochondrial DNA and RNA fragments from autophagic vacuoles , and insertion of mitochondrial DNA sequences , in some instances after reverse transcription of mitochondrial RNA , into the nuclear genome .
	manualset3
109144	18	403003	5	NULL	NULL	0	NULL	reverse transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Models are presented that describe mechanisms for the transfer of mitochondrial DNA into the nucleus involving fragmentation of mitochondrial DNA through aging and/or oxidative damage , anomalous processing or escape of mitochondrial DNA and RNA fragments from autophagic vacuoles , and insertion of mitochondrial DNA sequences , in some instances after reverse transcription of mitochondrial RNA , into the nuclear genome .
	manualset3
109145	19	403003	5	NULL	NULL	0	NULL	mitochondrial RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Models are presented that describe mechanisms for the transfer of mitochondrial DNA into the nucleus involving fragmentation of mitochondrial DNA through aging and/or oxidative damage , anomalous processing or escape of mitochondrial DNA and RNA fragments from autophagic vacuoles , and insertion of mitochondrial DNA sequences , in some instances after reverse transcription of mitochondrial RNA , into the nuclear genome .
	manualset3
109146	20	403003	5	NULL	NULL	0	NULL	nuclear genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Models are presented that describe mechanisms for the transfer of mitochondrial DNA into the nucleus involving fragmentation of mitochondrial DNA through aging and/or oxidative damage , anomalous processing or escape of mitochondrial DNA and RNA fragments from autophagic vacuoles , and insertion of mitochondrial DNA sequences , in some instances after reverse transcription of mitochondrial RNA , into the nuclear genome .
	manualset3
109182	1	403004	5	NULL	NULL	0	NULL	Models 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Models of CO2 concentrating mechanisms in microalgae taking into account cell and chloroplast structure .
	manualset3
109183	2	403004	5	NULL	NULL	0	NULL	CO2 concentrating mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Models of CO2 concentrating mechanisms in microalgae taking into account cell and chloroplast structure .
	manualset3
109184	3	403004	5	NULL	NULL	0	NULL	microalgae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Models of CO2 concentrating mechanisms in microalgae taking into account cell and chloroplast structure .
	manualset3
109185	4	403004	5	NULL	NULL	0	NULL	cell structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Models of CO2 concentrating mechanisms in microalgae taking into account cell and chloroplast structure .
	manualset3
109186	5	403004	5	NULL	NULL	0	NULL	chloroplast structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Models of CO2 concentrating mechanisms in microalgae taking into account cell and chloroplast structure .
	manualset3
109187	1	403005	5	NULL	NULL	0	NULL	Models 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Models of aldosterone action on sodium transport : emerging concepts .
	manualset3
109188	2	403005	5	NULL	NULL	0	NULL	aldosterone action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Models of aldosterone action on sodium transport : emerging concepts .
	manualset3
109189	3	403005	5	NULL	NULL	0	NULL	sodium transport	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Models of aldosterone action on sodium transport : emerging concepts .
	manualset3
109190	4	403005	5	NULL	NULL	0	NULL	emerging concepts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Models of aldosterone action on sodium transport : emerging concepts .
	manualset3
109191	1	403006	5	NULL	NULL	0	NULL	Models 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Models of cellular response provide a means of attempting to establish this connection .
	manualset3
109192	2	403006	5	NULL	NULL	0	NULL	cellular response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Models of cellular response provide a means of attempting to establish this connection .
	manualset3
109194	3	403006	5	NULL	NULL	NULL	NULL	connection	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Models of cellular response provide a means of attempting to establish this connection .
	manualset3
109195	1	403007	5	NULL	NULL	0	NULL	Moderate Na restriction	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Moderate Na restriction improved the consequences of nephron loss and restored the anti-hypertensive effect of drugs .
	manualset3
109196	2	403007	5	NULL	NULL	0	NULL	consequences 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Moderate Na restriction improved the consequences of nephron loss and restored the anti-hypertensive effect of drugs .
	manualset3
109197	3	403007	5	NULL	NULL	0	NULL	nephron loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Moderate Na restriction improved the consequences of nephron loss and restored the anti-hypertensive effect of drugs .
	manualset3
109198	4	403007	5	NULL	NULL	0	NULL	anti-hypertensive effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Moderate Na restriction improved the consequences of nephron loss and restored the anti-hypertensive effect of drugs .
	manualset3
109199	5	403007	5	NULL	NULL	0	NULL	drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Moderate Na restriction improved the consequences of nephron loss and restored the anti-hypertensive effect of drugs .
	manualset3
109201	1	403008	5	NULL	NULL	0	NULL	Moderator analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moderator analyses showed that the effects of the IYBP intervention on the primary child outcomes were not moderated by child or family demographic characteristics or risk factors .
	manualset3
109203	2	403008	5	NULL	NULL	0	NULL	IYBP intervention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Moderator analyses showed that the effects of the IYBP intervention on the primary child outcomes were not moderated by child or family demographic characteristics or risk factors .
	manualset3
109205	3	403008	5	NULL	NULL	0	NULL	primary child outcomes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moderator analyses showed that the effects of the IYBP intervention on the primary child outcomes were not moderated by child or family demographic characteristics or risk factors .
	manualset3
109206	4	403008	5	NULL	NULL	0	NULL	child 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Moderator analyses showed that the effects of the IYBP intervention on the primary child outcomes were not moderated by child or family demographic characteristics or risk factors .
	manualset3
109212	5	403008	5	NULL	NULL	0	NULL	family 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moderator analyses showed that the effects of the IYBP intervention on the primary child outcomes were not moderated by child or family demographic characteristics or risk factors .
	manualset3
109213	6	403008	5	NULL	NULL	NULL	NULL	demographic characteristics	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Moderator analyses showed that the effects of the IYBP intervention on the primary child outcomes were not moderated by child or family demographic characteristics or risk factors .
	manualset3
109214	7	403008	5	NULL	NULL	0	NULL	risk factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moderator analyses showed that the effects of the IYBP intervention on the primary child outcomes were not moderated by child or family demographic characteristics or risk factors .
	manualset3
109215	1	403009	5	NULL	NULL	NULL	NULL	Modern imaging techniques	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Modern imaging techniques now provide exact preoperative analyses , especially for orbital disorders .
	manualset3
109216	2	403009	5	NULL	NULL	0	NULL	preoperative analyses	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Modern imaging techniques now provide exact preoperative analyses , especially for orbital disorders .
	manualset3
109217	3	403009	5	NULL	NULL	0	NULL	orbital disorders 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Modern imaging techniques now provide exact preoperative analyses , especially for orbital disorders .
	manualset3
109218	1	403010	5	NULL	NULL	0	NULL	Modern methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Modern methods for investigating intercellular metabolic communication might help understanding the selective vulnerability seen in the basal ganglia of patients suffering from such neurodegenerative disorders in near future .
	manualset3
109219	2	403010	5	NULL	NULL	0	NULL	intercellular metabolic communication	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Modern methods for investigating intercellular metabolic communication might help understanding the selective vulnerability seen in the basal ganglia of patients suffering from such neurodegenerative disorders in near future .
	manualset3
109220	3	403010	5	NULL	NULL	0	NULL	selective vulnerability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modern methods for investigating intercellular metabolic communication might help understanding the selective vulnerability seen in the basal ganglia of patients suffering from such neurodegenerative disorders in near future .
	manualset3
109221	4	403010	5	NULL	NULL	0	NULL	basal ganglia	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Modern methods for investigating intercellular metabolic communication might help understanding the selective vulnerability seen in the basal ganglia of patients suffering from such neurodegenerative disorders in near future .
	manualset3
109222	5	403010	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Modern methods for investigating intercellular metabolic communication might help understanding the selective vulnerability seen in the basal ganglia of patients suffering from such neurodegenerative disorders in near future .
	manualset3
109223	6	403010	5	NULL	NULL	0	NULL	neurodegenerative disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Modern methods for investigating intercellular metabolic communication might help understanding the selective vulnerability seen in the basal ganglia of patients suffering from such neurodegenerative disorders in near future .
	manualset3
109224	7	403010	5	NULL	NULL	0	NULL	near future 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Modern methods for investigating intercellular metabolic communication might help understanding the selective vulnerability seen in the basal ganglia of patients suffering from such neurodegenerative disorders in near future .
	manualset3
109225	1	403011	5	NULL	NULL	0	NULL	Modern technology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Modern technology and advancement of knowledge in neurosurgery and interventional neuroradiology have altered its natural course for the better .
	manualset3
109226	2	403011	5	NULL	NULL	0	NULL	advancement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modern technology and advancement of knowledge in neurosurgery and interventional neuroradiology have altered its natural course for the better .
	manualset3
109227	3	403011	5	NULL	NULL	0	NULL	knowledge 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Modern technology and advancement of knowledge in neurosurgery and interventional neuroradiology have altered its natural course for the better .
	manualset3
109228	4	403011	5	NULL	NULL	0	NULL	neurosurgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Modern technology and advancement of knowledge in neurosurgery and interventional neuroradiology have altered its natural course for the better .
	manualset3
109229	5	403011	5	NULL	NULL	NULL	NULL	interventional neuroradiology	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Modern technology and advancement of knowledge in neurosurgery and interventional neuroradiology have altered its natural course for the better .
	manualset3
109230	6	403011	5	NULL	NULL	0	NULL	natural course	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modern technology and advancement of knowledge in neurosurgery and interventional neuroradiology have altered its natural course for the better .
	manualset3
109231	1	403012	5	NULL	NULL	0	NULL	case 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of conduction aphasia .
	manualset3
109232	2	403012	5	NULL	NULL	0	NULL	conduction aphasia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of conduction aphasia .
	manualset3
109233	1	403013	5	NULL	NULL	0	NULL	Modes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modes occurred sequentially in random order during GV first , with the same order then repeated during PLV .
	manualset3
109234	2	403013	5	NULL	NULL	0	NULL	random order	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modes occurred sequentially in random order during GV first , with the same order then repeated during PLV .
	manualset3
109235	3	403013	5	NULL	NULL	0	NULL	GV	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Modes occurred sequentially in random order during GV first , with the same order then repeated during PLV .
	manualset3
109236	4	403013	5	NULL	NULL	NULL	NULL	order 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Modes occurred sequentially in random order during GV first , with the same order then repeated during PLV .
	manualset3
109237	5	403013	5	NULL	NULL	0	NULL	PLV 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Modes occurred sequentially in random order during GV first , with the same order then repeated during PLV .
	manualset3
109238	1	403014	5	NULL	NULL	0	NULL	Modification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modification of fibrin network ultrastructure by Fab fragments specific for different domain of fibrinogen .
	manualset3
109239	2	403014	5	NULL	NULL	0	NULL	fibrin network ultrastructure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Modification of fibrin network ultrastructure by Fab fragments specific for different domain of fibrinogen .
	manualset3
109242	3	403014	5	NULL	NULL	0	NULL	Fab fragments 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Modification of fibrin network ultrastructure by Fab fragments specific for different domain of fibrinogen .
	manualset3
109244	4	403014	5	NULL	NULL	0	NULL	domain 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Modification of fibrin network ultrastructure by Fab fragments specific for different domain of fibrinogen .
	manualset3
109246	5	403014	5	NULL	NULL	0	NULL	fibrinogen 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Modification of fibrin network ultrastructure by Fab fragments specific for different domain of fibrinogen .
	manualset3
109247	1	403015	5	NULL	NULL	0	NULL	Modification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modification of protein to AGE/ALEs is known to be site-directed and this has potential implications for protein functionality and design of AGE/ALE inhibitors .
	manualset3
109248	2	403015	5	NULL	NULL	0	NULL	protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Modification of protein to AGE/ALEs is known to be site-directed and this has potential implications for protein functionality and design of AGE/ALE inhibitors .
	manualset3
109250	3	403015	5	NULL	NULL	0	NULL	AGE/ALEs 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Modification of protein to AGE/ALEs is known to be site-directed and this has potential implications for protein functionality and design of AGE/ALE inhibitors .
	manualset3
109251	4	403015	5	NULL	NULL	0	NULL	potential implications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modification of protein to AGE/ALEs is known to be site-directed and this has potential implications for protein functionality and design of AGE/ALE inhibitors .
	manualset3
109252	5	403015	5	NULL	NULL	0	NULL	protein functionality	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modification of protein to AGE/ALEs is known to be site-directed and this has potential implications for protein functionality and design of AGE/ALE inhibitors .
	manualset3
109253	6	403015	5	NULL	NULL	0	NULL	design 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modification of protein to AGE/ALEs is known to be site-directed and this has potential implications for protein functionality and design of AGE/ALE inhibitors .
	manualset3
109254	7	403015	5	NULL	NULL	NULL	NULL	AGE/ALE inhibitors	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Modification of protein to AGE/ALEs is known to be site-directed and this has potential implications for protein functionality and design of AGE/ALE inhibitors .
	manualset3
109255	1	403016	5	NULL	NULL	0	NULL	Modification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modification of the sinus node function is a new method of nonpharmacological treatments , although the skillfull and troublesome technique is required .
	manualset3
109256	2	403016	5	NULL	NULL	0	NULL	sinus node function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modification of the sinus node function is a new method of nonpharmacological treatments , although the skillfull and troublesome technique is required .
	manualset3
109257	3	403016	5	NULL	NULL	0	NULL	new method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Modification of the sinus node function is a new method of nonpharmacological treatments , although the skillfull and troublesome technique is required .
	manualset3
109258	4	403016	5	NULL	NULL	0	NULL	nonpharmacological treatments	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Modification of the sinus node function is a new method of nonpharmacological treatments , although the skillfull and troublesome technique is required .
	manualset3
109259	5	403016	5	NULL	NULL	0	NULL	skillfull technique 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Modification of the sinus node function is a new method of nonpharmacological treatments , although the skillfull and troublesome technique is required .
	manualset3
109261	6	403016	5	NULL	NULL	0	NULL	troublesome technique	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Modification of the sinus node function is a new method of nonpharmacological treatments , although the skillfull and troublesome technique is required .
	manualset3
109263	1	403017	5	NULL	NULL	0	NULL	Modifications 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modifications of hAPP introns 6 , 7 , and 8 in the PDGF-hAPP construct resulted in a prominent change in alternative splice site selection with transcripts encoding hAPP770 or hAPP751 being expressed at substantially higher levels than hAPP695 mRNA .
	manualset3
109267	2	403017	5	NULL	NULL	0	NULL	hAPP intron 6	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Modifications of hAPP introns 6 , 7 , and 8 in the PDGF-hAPP construct resulted in a prominent change in alternative splice site selection with transcripts encoding hAPP770 or hAPP751 being expressed at substantially higher levels than hAPP695 mRNA .
	manualset3
109269	3	403017	5	NULL	NULL	0	NULL	hAPP intron 7	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Modifications of hAPP introns 6 , 7 , and 8 in the PDGF-hAPP construct resulted in a prominent change in alternative splice site selection with transcripts encoding hAPP770 or hAPP751 being expressed at substantially higher levels than hAPP695 mRNA .
	manualset3
109271	4	403017	5	NULL	NULL	0	NULL	hAPP intron 8	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Modifications of hAPP introns 6 , 7 , and 8 in the PDGF-hAPP construct resulted in a prominent change in alternative splice site selection with transcripts encoding hAPP770 or hAPP751 being expressed at substantially higher levels than hAPP695 mRNA .
	manualset3
109273	5	403017	5	NULL	NULL	0	NULL	PDGF-hAPP construct	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Modifications of hAPP introns 6 , 7 , and 8 in the PDGF-hAPP construct resulted in a prominent change in alternative splice site selection with transcripts encoding hAPP770 or hAPP751 being expressed at substantially higher levels than hAPP695 mRNA .
	manualset3
109274	6	403017	5	NULL	NULL	0	NULL	prominent change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modifications of hAPP introns 6 , 7 , and 8 in the PDGF-hAPP construct resulted in a prominent change in alternative splice site selection with transcripts encoding hAPP770 or hAPP751 being expressed at substantially higher levels than hAPP695 mRNA .
	manualset3
109275	7	403017	5	NULL	NULL	0	NULL	alternative splice site selection	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Modifications of hAPP introns 6 , 7 , and 8 in the PDGF-hAPP construct resulted in a prominent change in alternative splice site selection with transcripts encoding hAPP770 or hAPP751 being expressed at substantially higher levels than hAPP695 mRNA .
	manualset3
109276	8	403017	5	NULL	NULL	0	NULL	transcripts 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Modifications of hAPP introns 6 , 7 , and 8 in the PDGF-hAPP construct resulted in a prominent change in alternative splice site selection with transcripts encoding hAPP770 or hAPP751 being expressed at substantially higher levels than hAPP695 mRNA .
	manualset3
109278	9	403017	5	NULL	NULL	0	NULL	hAPP770 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Modifications of hAPP introns 6 , 7 , and 8 in the PDGF-hAPP construct resulted in a prominent change in alternative splice site selection with transcripts encoding hAPP770 or hAPP751 being expressed at substantially higher levels than hAPP695 mRNA .
	manualset3
109279	10	403017	5	NULL	NULL	0	NULL	hAPP751 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Modifications of hAPP introns 6 , 7 , and 8 in the PDGF-hAPP construct resulted in a prominent change in alternative splice site selection with transcripts encoding hAPP770 or hAPP751 being expressed at substantially higher levels than hAPP695 mRNA .
	manualset3
109280	11	403017	5	NULL	NULL	0	NULL	higher levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Modifications of hAPP introns 6 , 7 , and 8 in the PDGF-hAPP construct resulted in a prominent change in alternative splice site selection with transcripts encoding hAPP770 or hAPP751 being expressed at substantially higher levels than hAPP695 mRNA .
	manualset3
109281	12	403017	5	NULL	NULL	0	NULL	hAPP695 mRNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Modifications of hAPP introns 6 , 7 , and 8 in the PDGF-hAPP construct resulted in a prominent change in alternative splice site selection with transcripts encoding hAPP770 or hAPP751 being expressed at substantially higher levels than hAPP695 mRNA .
	manualset3
109282	1	403018	5	NULL	NULL	NULL	NULL	Modifications 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Modifications of platelet functions by dietary fats .
	manualset3
109283	2	403018	5	NULL	NULL	NULL	NULL	platelet functions	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Modifications of platelet functions by dietary fats .
	manualset3
109288	3	403018	5	NULL	NULL	0	NULL	dietary fats	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Modifications of platelet functions by dietary fats .
	manualset3
109289	1	403019	5	NULL	NULL	0	NULL	Modifications 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modifications of typical asymmetric cortical patterns occur when pathology is present , as in hearing loss or tinnitus .
	manualset3
109290	2	403019	5	NULL	NULL	0	NULL	typical asymmetric cortical patterns	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modifications of typical asymmetric cortical patterns occur when pathology is present , as in hearing loss or tinnitus .
	manualset3
109291	3	403019	5	NULL	NULL	0	NULL	pathology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Modifications of typical asymmetric cortical patterns occur when pathology is present , as in hearing loss or tinnitus .
	manualset3
109292	4	403019	5	NULL	NULL	0	NULL	hearing loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Modifications of typical asymmetric cortical patterns occur when pathology is present , as in hearing loss or tinnitus .
	manualset3
109293	5	403019	5	NULL	NULL	0	NULL	tinnitus 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Modifications of typical asymmetric cortical patterns occur when pathology is present , as in hearing loss or tinnitus .
	manualset3
109294	1	403020	5	NULL	NULL	0	NULL	Modified abdominotransanal resection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Modified abdominotransanal resection for cancer of the lower third of the rectum .
	manualset3
109295	2	403020	5	NULL	NULL	0	NULL	cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Modified abdominotransanal resection for cancer of the lower third of the rectum .
	manualset3
109296	3	403020	5	NULL	NULL	NULL	NULL	rectum 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Modified abdominotransanal resection for cancer of the lower third of the rectum .
	manualset3
109297	1	403021	5	NULL	NULL	0	NULL	case 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of congenital intra-ocular tumor containing epithelium and cartilage .
	manualset3
109298	2	403021	5	NULL	NULL	0	NULL	congenital intra-ocular tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of congenital intra-ocular tumor containing epithelium and cartilage .
	manualset3
109299	3	403021	5	NULL	NULL	0	NULL	epithelium 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of congenital intra-ocular tumor containing epithelium and cartilage .
	manualset3
109300	4	403021	5	NULL	NULL	0	NULL	cartilage 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of congenital intra-ocular tumor containing epithelium and cartilage .
	manualset3
109309	1	403022	5	NULL	NULL	0	NULL	Modulation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of Wnt / - catenin signaling pathway by bioactive food components .
	manualset3
109310	2	403022	5	NULL	NULL	0	NULL	Wnt / - catenin signaling pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of Wnt / - catenin signaling pathway by bioactive food components .
	manualset3
109311	3	403022	5	NULL	NULL	0	NULL	bioactive food components	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of Wnt / - catenin signaling pathway by bioactive food components .
	manualset3
109312	1	403023	5	NULL	NULL	0	NULL	Modulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of a transient K + current in the pleural sensory neurons of Aplysia by serotonin and cAMP : implications for spike broadening .
	manualset3
109313	2	403023	5	NULL	NULL	NULL	NULL	transient K + current	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Modulation of a transient K + current in the pleural sensory neurons of Aplysia by serotonin and cAMP : implications for spike broadening .
	manualset3
109314	3	403023	5	NULL	NULL	0	NULL	pleural sensory neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of a transient K + current in the pleural sensory neurons of Aplysia by serotonin and cAMP : implications for spike broadening .
	manualset3
109315	4	403023	5	NULL	NULL	0	NULL	Aplysia 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of a transient K + current in the pleural sensory neurons of Aplysia by serotonin and cAMP : implications for spike broadening .
	manualset3
109316	5	403023	5	NULL	NULL	0	NULL	serotonin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of a transient K + current in the pleural sensory neurons of Aplysia by serotonin and cAMP : implications for spike broadening .
	manualset3
109317	6	403023	5	NULL	NULL	0	NULL	cAMP 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of a transient K + current in the pleural sensory neurons of Aplysia by serotonin and cAMP : implications for spike broadening .
	manualset3
109318	7	403023	5	NULL	NULL	0	NULL	implications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of a transient K + current in the pleural sensory neurons of Aplysia by serotonin and cAMP : implications for spike broadening .
	manualset3
109319	8	403023	5	NULL	NULL	0	NULL	spike broadening	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of a transient K + current in the pleural sensory neurons of Aplysia by serotonin and cAMP : implications for spike broadening .
	manualset3
109320	1	403024	5	NULL	NULL	0	NULL	Modulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of angiogenesis during adipose tissue development in murine models of obesity .
	manualset3
109321	2	403024	5	NULL	NULL	0	NULL	angiogenesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of angiogenesis during adipose tissue development in murine models of obesity .
	manualset3
109322	3	403024	5	NULL	NULL	0	NULL	adipose tissue development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of angiogenesis during adipose tissue development in murine models of obesity .
	manualset3
109323	4	403024	5	NULL	NULL	0	NULL	murine models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of angiogenesis during adipose tissue development in murine models of obesity .
	manualset3
109324	5	403024	5	NULL	NULL	0	NULL	obesity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of angiogenesis during adipose tissue development in murine models of obesity .
	manualset3
109325	1	403025	5	NULL	NULL	0	NULL	Modulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of aromatase activity and expression by environmental chemicals .
	manualset3
109326	2	403025	5	NULL	NULL	0	NULL	aromatase activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of aromatase activity and expression by environmental chemicals .
	manualset3
109327	3	403025	5	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of aromatase activity and expression by environmental chemicals .
	manualset3
109328	4	403025	5	NULL	NULL	0	NULL	environmental chemicals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of aromatase activity and expression by environmental chemicals .
	manualset3
109329	1	403026	5	NULL	NULL	0	NULL	Modulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of experimental allergic encephalomyelitis in mice by immunization with a peptide specific for the gamma delta T cell receptor .
	manualset3
109330	2	403026	5	NULL	NULL	0	NULL	experimental allergic encephalomyelitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of experimental allergic encephalomyelitis in mice by immunization with a peptide specific for the gamma delta T cell receptor .
	manualset3
109331	3	403026	5	NULL	NULL	0	NULL	mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of experimental allergic encephalomyelitis in mice by immunization with a peptide specific for the gamma delta T cell receptor .
	manualset3
109332	4	403026	5	NULL	NULL	0	NULL	immunization 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of experimental allergic encephalomyelitis in mice by immunization with a peptide specific for the gamma delta T cell receptor .
	manualset3
109333	5	403026	5	NULL	NULL	0	NULL	peptide specific for the gamma delta T cell receptor	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of experimental allergic encephalomyelitis in mice by immunization with a peptide specific for the gamma delta T cell receptor .
	manualset3
109334	1	403027	5	NULL	NULL	0	NULL	Modulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of humoral immune response to influenza vaccines by BCG .
	manualset3
109335	2	403027	5	NULL	NULL	0	NULL	humoral immune response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of humoral immune response to influenza vaccines by BCG .
	manualset3
109336	3	403027	5	NULL	NULL	0	NULL	influenza vaccines	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of humoral immune response to influenza vaccines by BCG .
	manualset3
109337	4	403027	5	NULL	NULL	0	NULL	BCG	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of humoral immune response to influenza vaccines by BCG .
	manualset3
109338	1	403028	5	NULL	NULL	0	NULL	Modulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of lipase hydrolysis and synthesis reactions using carbohydrates .
	manualset3
109339	2	403028	5	NULL	NULL	0	NULL	lipase hydrolysis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of lipase hydrolysis and synthesis reactions using carbohydrates .
	manualset3
109340	3	403028	5	NULL	NULL	0	NULL	synthesis reactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of lipase hydrolysis and synthesis reactions using carbohydrates .
	manualset3
109341	4	403028	5	NULL	NULL	0	NULL	carbohydrates	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of lipase hydrolysis and synthesis reactions using carbohydrates .
	manualset3
109342	1	403029	5	NULL	NULL	0	NULL	Modulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of organ uptake of 11C-labelled L-DOPA .
	manualset3
109343	2	403029	5	NULL	NULL	0	NULL	organ uptake	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of organ uptake of 11C-labelled L-DOPA .
	manualset3
109344	3	403029	5	NULL	NULL	0	NULL	11C-labelled L-DOPA	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of organ uptake of 11C-labelled L-DOPA .
	manualset3
109345	1	403030	5	NULL	NULL	0	NULL	Modulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of perineuronal nets and parvalbumin with developmental song learning .
	manualset3
109346	2	403030	5	NULL	NULL	NULL	NULL	Perineuronal net	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Modulation of perineuronal nets and parvalbumin with developmental song learning .
	manualset3
109347	3	403030	5	NULL	NULL	0	NULL	parvalbumin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of perineuronal nets and parvalbumin with developmental song learning .
	manualset3
109348	4	403030	5	NULL	NULL	0	NULL	developmental song learning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of perineuronal nets and parvalbumin with developmental song learning .
	manualset3
109477	1	403031	5	NULL	NULL	0	NULL	Modulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of polyglutamine conformations and dimer formation by the N-terminus of huntingtin .
	manualset3
109478	2	403031	5	NULL	NULL	NULL	NULL	polyglutamine conformations	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Modulation of polyglutamine conformations and dimer formation by the N-terminus of huntingtin .
	manualset3
109479	3	403031	5	NULL	NULL	0	NULL	dimer formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of polyglutamine conformations and dimer formation by the N-terminus of huntingtin .
	manualset3
109480	4	403031	5	NULL	NULL	0	NULL	N-terminus	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of polyglutamine conformations and dimer formation by the N-terminus of huntingtin .
	manualset3
109481	5	403031	5	NULL	NULL	NULL	NULL	huntingtin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Modulation of polyglutamine conformations and dimer formation by the N-terminus of huntingtin .
	manualset3
109482	1	403032	5	NULL	NULL	0	NULL	Modulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of vascular cyclic nucleotide phosphodiesterases by cyclic GMP : role in vasodilatation .
	manualset3
109483	2	403032	5	NULL	NULL	0	NULL	vascular cyclic nucleotide phosphodiesterases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of vascular cyclic nucleotide phosphodiesterases by cyclic GMP : role in vasodilatation .
	manualset3
109484	3	403032	5	NULL	NULL	0	NULL	cyclic GMP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of vascular cyclic nucleotide phosphodiesterases by cyclic GMP : role in vasodilatation .
	manualset3
109485	4	403032	5	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of vascular cyclic nucleotide phosphodiesterases by cyclic GMP : role in vasodilatation .
	manualset3
109486	5	403032	5	NULL	NULL	0	NULL	vasodilatation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Modulation of vascular cyclic nucleotide phosphodiesterases by cyclic GMP : role in vasodilatation .
	manualset3
109487	1	403033	5	NULL	NULL	0	NULL	Molecular-genetic approaches	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular-genetic approaches to the classification of animals .
	manualset3
109488	2	403033	5	NULL	NULL	0	NULL	classification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular-genetic approaches to the classification of animals .
	manualset3
109489	3	403033	5	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular-genetic approaches to the classification of animals .
	manualset3
109490	1	403034	5	NULL	NULL	0	NULL	Molecular Body Imaging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular Body Imaging : MR Imaging , CT , and US .
	manualset3
109491	2	403034	5	NULL	NULL	0	NULL	MR Imaging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular Body Imaging : MR Imaging , CT , and US .
	manualset3
109492	3	403034	5	NULL	NULL	0	NULL	CT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular Body Imaging : MR Imaging , CT , and US .
	manualset3
109493	4	403034	5	NULL	NULL	0	NULL	US	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular Body Imaging : MR Imaging , CT , and US .
	manualset3
109494	1	403035	5	NULL	NULL	0	NULL	Molecular analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular analysis revealed a duplication at chromosome 17p11.2-12 , which is a known genetic cause of Charcot-Marie-Tooth disease type 1A ( CMT1A ) .
	manualset3
109495	2	403035	5	NULL	NULL	0	NULL	duplication	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular analysis revealed a duplication at chromosome 17p11.2-12 , which is a known genetic cause of Charcot-Marie-Tooth disease type 1A ( CMT1A ) .
	manualset3
109496	3	403035	5	NULL	NULL	0	NULL	chromosome 17p11.2-12 	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular analysis revealed a duplication at chromosome 17p11.2-12 , which is a known genetic cause of Charcot-Marie-Tooth disease type 1A ( CMT1A ) .
	manualset3
109497	4	403035	5	NULL	NULL	0	NULL	Charcot-Marie-Tooth disease type 1A ( CMT1A )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular analysis revealed a duplication at chromosome 17p11.2-12 , which is a known genetic cause of Charcot-Marie-Tooth disease type 1A ( CMT1A ) .
	manualset3
109502	1	403036	5	NULL	NULL	0	NULL	Molecular characterisation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular and genetic characterisation of the host-protective oncosphere antigens of taeniid cestode parasites .
	manualset3
109503	2	403036	5	NULL	NULL	0	NULL	genetic characterisation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular and genetic characterisation of the host-protective oncosphere antigens of taeniid cestode parasites .
	manualset3
109504	3	403036	5	NULL	NULL	0	NULL	host-protective oncosphere antigens	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular and genetic characterisation of the host-protective oncosphere antigens of taeniid cestode parasites .
	manualset3
109505	4	403036	5	NULL	NULL	0	NULL	taeniid cestode parasites	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular and genetic characterisation of the host-protective oncosphere antigens of taeniid cestode parasites .
	manualset3
109506	1	403037	5	NULL	NULL	0	NULL	HIV-1 protease	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular basis of HIV-1 protease drug resistance : structural analysis of mutant proteases complexed with cyclic urea inhibitors .
	manualset3
109507	2	403037	5	NULL	NULL	0	NULL	drug resistance	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular basis of HIV-1 protease drug resistance : structural analysis of mutant proteases complexed with cyclic urea inhibitors .
	manualset3
109533	3	403037	5	NULL	NULL	0	NULL	structural analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular basis of HIV-1 protease drug resistance : structural analysis of mutant proteases complexed with cyclic urea inhibitors .
	manualset3
109534	4	403037	5	NULL	NULL	0	NULL	mutant proteases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular basis of HIV-1 protease drug resistance : structural analysis of mutant proteases complexed with cyclic urea inhibitors .
	manualset3
109535	5	403037	5	NULL	NULL	0	NULL	cyclic urea inhibitors	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular basis of HIV-1 protease drug resistance : structural analysis of mutant proteases complexed with cyclic urea inhibitors .
	manualset3
109540	1	403038	5	NULL	NULL	0	NULL	black tea theaflavins	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular binding of black tea theaflavins to biological membranes : relationship to bioactivities .
	manualset3
109541	2	403038	5	NULL	NULL	0	NULL	biological membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular binding of black tea theaflavins to biological membranes : relationship to bioactivities .
	manualset3
109542	3	403038	5	NULL	NULL	0	NULL	relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular binding of black tea theaflavins to biological membranes : relationship to bioactivities .
	manualset3
109543	4	403038	5	NULL	NULL	0	NULL	bioactivities 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular binding of black tea theaflavins to biological membranes : relationship to bioactivities .
	manualset3
112975	5	403038	5	NULL	NULL	0	NULL	Molecular binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular binding of black tea theaflavins to biological membranes : relationship to bioactivities .
	manualset3
109544	1	403039	5	NULL	NULL	0	NULL	Molecular cloning 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular cloning of chick lysyl hydroxylase .
	manualset3
109546	2	403039	5	NULL	NULL	NULL	NULL	chick lysyl hydroxylase	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Molecular cloning of chick lysyl hydroxylase .
	manualset3
109547	1	403040	5	NULL	NULL	0	NULL	Molecular cloning	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular cloning of murine STAP-1 , the stem-cell-specific adaptor protein containing PH and SH2 domains .
	manualset3
109548	2	403040	5	NULL	NULL	NULL	NULL	murine STAP-1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Molecular cloning of murine STAP-1 , the stem-cell-specific adaptor protein containing PH and SH2 domains .
	manualset3
109549	3	403040	5	NULL	NULL	0	NULL	stem-cell-specific adaptor protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular cloning of murine STAP-1 , the stem-cell-specific adaptor protein containing PH and SH2 domains .
	manualset3
109550	4	403040	5	NULL	NULL	0	NULL	PH domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular cloning of murine STAP-1 , the stem-cell-specific adaptor protein containing PH and SH2 domains .
	manualset3
109551	5	403040	5	NULL	NULL	0	NULL	SH2 domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular cloning of murine STAP-1 , the stem-cell-specific adaptor protein containing PH and SH2 domains .
	manualset3
109552	1	403041	5	NULL	NULL	0	NULL	Molecular cloning	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular cloning of three types of arginine vasotocin receptor in the newt , Cynops pyrrhogaster .
	manualset3
109553	2	403041	5	NULL	NULL	0	NULL	three types	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular cloning of three types of arginine vasotocin receptor in the newt , Cynops pyrrhogaster .
	manualset3
109554	3	403041	5	NULL	NULL	0	NULL	arginine vasotocin receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular cloning of three types of arginine vasotocin receptor in the newt , Cynops pyrrhogaster .
	manualset3
109555	4	403041	5	NULL	NULL	0	NULL	newt , Cynops pyrrhogaster	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular cloning of three types of arginine vasotocin receptor in the newt , Cynops pyrrhogaster .
	manualset3
109556	1	403042	5	NULL	NULL	0	NULL	Molecular cytogenetic discrimination	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular cytogenetic discrimination and reaction to wheat streak mosaic virus and the wheat curl mite in Zhong series of wheat -- Thinopyrum intermedium partial amphiploids .
	manualset3
109557	2	403042	5	NULL	NULL	0	NULL	reaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular cytogenetic discrimination and reaction to wheat streak mosaic virus and the wheat curl mite in Zhong series of wheat -- Thinopyrum intermedium partial amphiploids .
	manualset3
109559	3	403042	5	NULL	NULL	0	NULL	wheat streak mosaic virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular cytogenetic discrimination and reaction to wheat streak mosaic virus and the wheat curl mite in Zhong series of wheat -- Thinopyrum intermedium partial amphiploids .
	manualset3
109560	4	403042	5	NULL	NULL	0	NULL	wheat curl mite	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular cytogenetic discrimination and reaction to wheat streak mosaic virus and the wheat curl mite in Zhong series of wheat -- Thinopyrum intermedium partial amphiploids .
	manualset3
109561	5	403042	5	NULL	NULL	0	NULL	Zhong series of wheat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular cytogenetic discrimination and reaction to wheat streak mosaic virus and the wheat curl mite in Zhong series of wheat -- Thinopyrum intermedium partial amphiploids .
	manualset3
109562	6	403042	5	NULL	NULL	0	NULL	Thinopyrum intermedium partial amphiploids	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular cytogenetic discrimination and reaction to wheat streak mosaic virus and the wheat curl mite in Zhong series of wheat -- Thinopyrum intermedium partial amphiploids .
	manualset3
109563	1	403043	5	NULL	NULL	NULL	NULL	Molecular detection	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Molecular detection of rabies encephalitis and correlation with cytokine expression .
	manualset3
109564	2	403043	5	NULL	NULL	0	NULL	rabies encephalitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular detection of rabies encephalitis and correlation with cytokine expression .
	manualset3
109565	3	403043	5	NULL	NULL	NULL	NULL	correlation 	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Molecular detection of rabies encephalitis and correlation with cytokine expression .
	manualset3
109566	4	403043	5	NULL	NULL	0	NULL	cytokine expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular detection of rabies encephalitis and correlation with cytokine expression .
	manualset3
109567	1	403044	5	NULL	NULL	0	NULL	Molecular detection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular detection or carriers of hemophilia A in Mexican families .
	manualset3
109568	2	403044	5	NULL	NULL	0	NULL	carriers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular detection or carriers of hemophilia A in Mexican families .
	manualset3
109569	3	403044	5	NULL	NULL	0	NULL	hemophilia A	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular detection or carriers of hemophilia A in Mexican families .
	manualset3
109570	4	403044	5	NULL	NULL	0	NULL	Mexican families	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular detection or carriers of hemophilia A in Mexican families .
	manualset3
109571	1	403045	5	NULL	NULL	0	NULL	Molecular docking study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular docking study sequentially elaborated the plausible binding modes of the structurally diverse sugar-based inhibitors with PTP1B .
	manualset3
109572	2	403045	5	NULL	NULL	0	NULL	binding modes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular docking study sequentially elaborated the plausible binding modes of the structurally diverse sugar-based inhibitors with PTP1B .
	manualset3
109573	3	403045	5	NULL	NULL	0	NULL	structurally diverse sugar-based inhibitors	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular docking study sequentially elaborated the plausible binding modes of the structurally diverse sugar-based inhibitors with PTP1B .
	manualset3
109574	4	403045	5	NULL	NULL	0	NULL	PTP1B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular docking study sequentially elaborated the plausible binding modes of the structurally diverse sugar-based inhibitors with PTP1B .
	manualset3
109575	1	403046	5	NULL	NULL	0	NULL	Molecular dynamics ( MD ) simulations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular dynamics ( MD ) simulations and ab initio quantum chemical calculations were employed to investigate the structure , dynamics and interactions of the QSY 21 nonfluorescent quencher and the fluorescence dye Rhodamine 6G bound to a B-DNA decamer .
	manualset3
109576	2	403046	5	NULL	NULL	0	NULL	ab initio quantum chemical calculations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular dynamics ( MD ) simulations and ab initio quantum chemical calculations were employed to investigate the structure , dynamics and interactions of the QSY 21 nonfluorescent quencher and the fluorescence dye Rhodamine 6G bound to a B-DNA decamer .
	manualset3
109577	3	403046	5	NULL	NULL	0	NULL	dynamics 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular dynamics ( MD ) simulations and ab initio quantum chemical calculations were employed to investigate the structure , dynamics and interactions of the QSY 21 nonfluorescent quencher and the fluorescence dye Rhodamine 6G bound to a B-DNA decamer .
	manualset3
109578	4	403046	5	NULL	NULL	0	NULL	interactions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular dynamics ( MD ) simulations and ab initio quantum chemical calculations were employed to investigate the structure , dynamics and interactions of the QSY 21 nonfluorescent quencher and the fluorescence dye Rhodamine 6G bound to a B-DNA decamer .
	manualset3
109579	5	403046	5	NULL	NULL	0	NULL	QSY 21 nonfluorescent quencher 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular dynamics ( MD ) simulations and ab initio quantum chemical calculations were employed to investigate the structure , dynamics and interactions of the QSY 21 nonfluorescent quencher and the fluorescence dye Rhodamine 6G bound to a B-DNA decamer .
	manualset3
109580	6	403046	5	NULL	NULL	0	NULL	fluorescence dye Rhodamine 6G	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular dynamics ( MD ) simulations and ab initio quantum chemical calculations were employed to investigate the structure , dynamics and interactions of the QSY 21 nonfluorescent quencher and the fluorescence dye Rhodamine 6G bound to a B-DNA decamer .
	manualset3
109581	7	403046	5	NULL	NULL	0	NULL	B-DNA decamer	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular dynamics ( MD ) simulations and ab initio quantum chemical calculations were employed to investigate the structure , dynamics and interactions of the QSY 21 nonfluorescent quencher and the fluorescence dye Rhodamine 6G bound to a B-DNA decamer .
	manualset3
109582	1	403047	5	NULL	NULL	0	NULL	Molecular dynamics simulations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular dynamics simulations have been performed for the uranyl ion and up to 400 water molecules .
	manualset3
109583	2	403047	5	NULL	NULL	0	NULL	uranyl ion	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular dynamics simulations have been performed for the uranyl ion and up to 400 water molecules .
	manualset3
109584	3	403047	5	NULL	NULL	0	NULL	400 water molecules	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular dynamics simulations have been performed for the uranyl ion and up to 400 water molecules .
	manualset3
109585	1	403048	5	NULL	NULL	0	NULL	Molecular dynamics simulations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular dynamics simulations of alpha-lytic protease ( alphaLP ) alone and complexed with its pro region ( PRO ) are performed to understand the origin of its high unfolding ( and folding ) barrier when it is alone and how the pro region lowers this barrier .
	manualset3
109586	2	403048	5	NULL	NULL	0	NULL	alpha-lytic protease ( alphaLP ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular dynamics simulations of alpha-lytic protease ( alphaLP ) alone and complexed with its pro region ( PRO ) are performed to understand the origin of its high unfolding ( and folding ) barrier when it is alone and how the pro region lowers this barrier .
	manualset3
109587	3	403048	5	NULL	NULL	0	NULL	pro region ( PRO )	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular dynamics simulations of alpha-lytic protease ( alphaLP ) alone and complexed with its pro region ( PRO ) are performed to understand the origin of its high unfolding ( and folding ) barrier when it is alone and how the pro region lowers this barrier .
	manualset3
109588	4	403048	5	NULL	NULL	0	NULL	origin 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular dynamics simulations of alpha-lytic protease ( alphaLP ) alone and complexed with its pro region ( PRO ) are performed to understand the origin of its high unfolding ( and folding ) barrier when it is alone and how the pro region lowers this barrier .
	manualset3
109589	5	403048	5	NULL	NULL	0	NULL	high unfolding ( and folding ) barrier	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular dynamics simulations of alpha-lytic protease ( alphaLP ) alone and complexed with its pro region ( PRO ) are performed to understand the origin of its high unfolding ( and folding ) barrier when it is alone and how the pro region lowers this barrier .
	manualset3
109590	6	403048	5	NULL	NULL	0	NULL	pro region	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular dynamics simulations of alpha-lytic protease ( alphaLP ) alone and complexed with its pro region ( PRO ) are performed to understand the origin of its high unfolding ( and folding ) barrier when it is alone and how the pro region lowers this barrier .
	manualset3
109591	7	403048	5	NULL	NULL	0	NULL	barrier 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular dynamics simulations of alpha-lytic protease ( alphaLP ) alone and complexed with its pro region ( PRO ) are performed to understand the origin of its high unfolding ( and folding ) barrier when it is alone and how the pro region lowers this barrier .
	manualset3
109592	1	403049	5	NULL	NULL	0	NULL	Molecular electrostatic potential ( MEP ) calculations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular electrostatic potential ( MEP ) calculations using ab initio SCF methods ranging from 3-21G to 6-31G levels have been performed to visualize their three-dimensional pharmacophoric patterns and topography .
	manualset3
109593	2	403049	5	NULL	NULL	0	NULL	ab initio SCF methods	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular electrostatic potential ( MEP ) calculations using ab initio SCF methods ranging from 3-21G to 6-31G levels have been performed to visualize their three-dimensional pharmacophoric patterns and topography .
	manualset3
109594	3	403049	5	NULL	NULL	0	NULL	 3-21G to 6-31G levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular electrostatic potential ( MEP ) calculations using ab initio SCF methods ranging from 3-21G to 6-31G levels have been performed to visualize their three-dimensional pharmacophoric patterns and topography .
	manualset3
109595	4	403049	5	NULL	NULL	0	NULL	three-dimensional pharmacophoric patterns	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular electrostatic potential ( MEP ) calculations using ab initio SCF methods ranging from 3-21G to 6-31G levels have been performed to visualize their three-dimensional pharmacophoric patterns and topography .
	manualset3
109596	5	403049	5	NULL	NULL	0	NULL	topography 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular electrostatic potential ( MEP ) calculations using ab initio SCF methods ranging from 3-21G to 6-31G levels have been performed to visualize their three-dimensional pharmacophoric patterns and topography .
	manualset3
109597	1	403050	5	NULL	NULL	0	NULL	Molecular epidemiology studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular epidemiology studies suggested that the sudden worldwide increase of CTX-M-15-producing E. coli is mostly due to a single clone named ST131 and that foreign travel to high-risk areas such as the Indian subcontinent might in part play a role in the spread of this clone across different continents .
	manualset3
109598	2	403050	5	NULL	NULL	0	NULL	CTX-M-15-producing E. coli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular epidemiology studies suggested that the sudden worldwide increase of CTX-M-15-producing E. coli is mostly due to a single clone named ST131 and that foreign travel to high-risk areas such as the Indian subcontinent might in part play a role in the spread of this clone across different continents .
	manualset3
109599	3	403050	5	NULL	NULL	0	NULL	single clone 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular epidemiology studies suggested that the sudden worldwide increase of CTX-M-15-producing E. coli is mostly due to a single clone named ST131 and that foreign travel to high-risk areas such as the Indian subcontinent might in part play a role in the spread of this clone across different continents .
	manualset3
109600	4	403050	5	NULL	NULL	0	NULL	ST131 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular epidemiology studies suggested that the sudden worldwide increase of CTX-M-15-producing E. coli is mostly due to a single clone named ST131 and that foreign travel to high-risk areas such as the Indian subcontinent might in part play a role in the spread of this clone across different continents .
	manualset3
109601	5	403050	5	NULL	NULL	0	NULL	foreign travel 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular epidemiology studies suggested that the sudden worldwide increase of CTX-M-15-producing E. coli is mostly due to a single clone named ST131 and that foreign travel to high-risk areas such as the Indian subcontinent might in part play a role in the spread of this clone across different continents .
	manualset3
109602	6	403050	5	NULL	NULL	0	NULL	high-risk areas	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular epidemiology studies suggested that the sudden worldwide increase of CTX-M-15-producing E. coli is mostly due to a single clone named ST131 and that foreign travel to high-risk areas such as the Indian subcontinent might in part play a role in the spread of this clone across different continents .
	manualset3
109603	7	403050	5	NULL	NULL	0	NULL	Indian subcontinent 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular epidemiology studies suggested that the sudden worldwide increase of CTX-M-15-producing E. coli is mostly due to a single clone named ST131 and that foreign travel to high-risk areas such as the Indian subcontinent might in part play a role in the spread of this clone across different continents .
	manualset3
109604	8	403050	5	NULL	NULL	0	NULL	play a role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular epidemiology studies suggested that the sudden worldwide increase of CTX-M-15-producing E. coli is mostly due to a single clone named ST131 and that foreign travel to high-risk areas such as the Indian subcontinent might in part play a role in the spread of this clone across different continents .
	manualset3
109605	9	403050	5	NULL	NULL	0	NULL	spread 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular epidemiology studies suggested that the sudden worldwide increase of CTX-M-15-producing E. coli is mostly due to a single clone named ST131 and that foreign travel to high-risk areas such as the Indian subcontinent might in part play a role in the spread of this clone across different continents .
	manualset3
109606	10	403050	5	NULL	NULL	0	NULL	clone 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular epidemiology studies suggested that the sudden worldwide increase of CTX-M-15-producing E. coli is mostly due to a single clone named ST131 and that foreign travel to high-risk areas such as the Indian subcontinent might in part play a role in the spread of this clone across different continents .
	manualset3
109607	11	403050	5	NULL	NULL	0	NULL	different continents 	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular epidemiology studies suggested that the sudden worldwide increase of CTX-M-15-producing E. coli is mostly due to a single clone named ST131 and that foreign travel to high-risk areas such as the Indian subcontinent might in part play a role in the spread of this clone across different continents .
	manualset3
109658	1	403051	5	NULL	NULL	0	NULL	Molecular evidence	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular evidence of a unique lipoamide dehydrogenase in plastids : analysis of plastidic lipoamide dehydrogenase from Arabidopsis thaliana .
	manualset3
109659	2	403051	5	NULL	NULL	0	NULL	 lipoamide dehydrogenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular evidence of a unique lipoamide dehydrogenase in plastids : analysis of plastidic lipoamide dehydrogenase from Arabidopsis thaliana .
	manualset3
109660	3	403051	5	NULL	NULL	0	NULL	plastids	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular evidence of a unique lipoamide dehydrogenase in plastids : analysis of plastidic lipoamide dehydrogenase from Arabidopsis thaliana .
	manualset3
109661	4	403051	5	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular evidence of a unique lipoamide dehydrogenase in plastids : analysis of plastidic lipoamide dehydrogenase from Arabidopsis thaliana .
	manualset3
109662	5	403051	5	NULL	NULL	0	NULL	plastidic lipoamide dehydrogenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular evidence of a unique lipoamide dehydrogenase in plastids : analysis of plastidic lipoamide dehydrogenase from Arabidopsis thaliana .
	manualset3
109663	6	403051	5	NULL	NULL	0	NULL	Arabidopsis thaliana 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular evidence of a unique lipoamide dehydrogenase in plastids : analysis of plastidic lipoamide dehydrogenase from Arabidopsis thaliana .
	manualset3
109664	1	403052	5	NULL	NULL	0	NULL	Molecular evolution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular evolution of amelogenin in mammals .
	manualset3
109665	2	403052	5	NULL	NULL	0	NULL	amelogenin	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular evolution of amelogenin in mammals .
	manualset3
109666	3	403052	5	NULL	NULL	0	NULL	mammals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular evolution of amelogenin in mammals .
	manualset3
110865	1	403053	5	NULL	NULL	0	NULL	Molecular formulas	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular formulas C28H46N4O6 , C27H44N4O6 and C26H42N4O6 for cepafungins I , II and III were indicated by elemental analysis and SI-MS .
	manualset3
110866	2	403053	5	NULL	NULL	0	NULL	C28H46N4O6	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular formulas C28H46N4O6 , C27H44N4O6 and C26H42N4O6 for cepafungins I , II and III were indicated by elemental analysis and SI-MS .
	manualset3
110867	3	403053	5	NULL	NULL	0	NULL	C27H44N4O6	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular formulas C28H46N4O6 , C27H44N4O6 and C26H42N4O6 for cepafungins I , II and III were indicated by elemental analysis and SI-MS .
	manualset3
110868	4	403053	5	NULL	NULL	0	NULL	C26H42N4O6	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular formulas C28H46N4O6 , C27H44N4O6 and C26H42N4O6 for cepafungins I , II and III were indicated by elemental analysis and SI-MS .
	manualset3
110869	5	403053	5	NULL	NULL	0	NULL	cepafungin I 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular formulas C28H46N4O6 , C27H44N4O6 and C26H42N4O6 for cepafungins I , II and III were indicated by elemental analysis and SI-MS .
	manualset3
110870	6	403053	5	NULL	NULL	0	NULL	cepafungin II	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular formulas C28H46N4O6 , C27H44N4O6 and C26H42N4O6 for cepafungins I , II and III were indicated by elemental analysis and SI-MS .
	manualset3
110871	7	403053	5	NULL	NULL	0	NULL	cepafungin III	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular formulas C28H46N4O6 , C27H44N4O6 and C26H42N4O6 for cepafungins I , II and III were indicated by elemental analysis and SI-MS .
	manualset3
110872	8	403053	5	NULL	NULL	0	NULL	elemental analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular formulas C28H46N4O6 , C27H44N4O6 and C26H42N4O6 for cepafungins I , II and III were indicated by elemental analysis and SI-MS .
	manualset3
110873	9	403053	5	NULL	NULL	0	NULL	SI-MS	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular formulas C28H46N4O6 , C27H44N4O6 and C26H42N4O6 for cepafungins I , II and III were indicated by elemental analysis and SI-MS .
	manualset3
109667	1	403054	5	NULL	NULL	0	NULL	Molecular genetic aspects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular genetic aspects of sex determination in Drosophila melanogaster .
	manualset3
109668	2	403054	5	NULL	NULL	0	NULL	sex determination	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular genetic aspects of sex determination in Drosophila melanogaster .
	manualset3
109669	3	403054	5	NULL	NULL	0	NULL	Drosophila melanogaster	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular genetic aspects of sex determination in Drosophila melanogaster .
	manualset3
109670	1	403055	5	NULL	NULL	0	NULL	case	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of group D xeroderma pigmentosum is reported .
	manualset3
109671	2	403055	5	NULL	NULL	0	NULL	group D xeroderma pigmentosum	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of group D xeroderma pigmentosum is reported .
	manualset3
109672	1	403056	5	NULL	NULL	0	NULL	Molecular insights	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular insights on the two fluorescence lifetimes displayed by warfarin from fluorescence anisotropy and molecular dynamics studies .
	manualset3
109673	2	403056	5	NULL	NULL	0	NULL	two fluorescence lifetimes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular insights on the two fluorescence lifetimes displayed by warfarin from fluorescence anisotropy and molecular dynamics studies .
	manualset3
109674	3	403056	5	NULL	NULL	0	NULL	warfarin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular insights on the two fluorescence lifetimes displayed by warfarin from fluorescence anisotropy and molecular dynamics studies .
	manualset3
109675	4	403056	5	NULL	NULL	0	NULL	fluorescence anisotropy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular insights on the two fluorescence lifetimes displayed by warfarin from fluorescence anisotropy and molecular dynamics studies .
	manualset3
109676	5	403056	5	NULL	NULL	0	NULL	molecular dynamics studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular insights on the two fluorescence lifetimes displayed by warfarin from fluorescence anisotropy and molecular dynamics studies .
	manualset3
109677	1	403057	5	NULL	NULL	0	NULL	Molecular mimicry	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular mimicry and antigen-specific T cell responses in multiple sclerosis and chronic CNS Lyme disease .
	manualset3
109678	2	403057	5	NULL	NULL	0	NULL	antigen-specific T cell responses	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular mimicry and antigen-specific T cell responses in multiple sclerosis and chronic CNS Lyme disease .
	manualset3
109679	3	403057	5	NULL	NULL	0	NULL	multiple sclerosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular mimicry and antigen-specific T cell responses in multiple sclerosis and chronic CNS Lyme disease .
	manualset3
109680	4	403057	5	NULL	NULL	0	NULL	chronic CNS Lyme disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular mimicry and antigen-specific T cell responses in multiple sclerosis and chronic CNS Lyme disease .
	manualset3
109681	1	403058	5	NULL	NULL	0	NULL	Molecular modelling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular modelling suggests that this built-in arginine mimics the catalytic arginine residues found in trimeric GTPases and GTPase-activating proteins in providing the positive charge to facilitate the GTP hydrolysis reaction .
	manualset3
109682	2	403058	5	NULL	NULL	0	NULL	built-in arginine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular modelling suggests that this built-in arginine mimics the catalytic arginine residues found in trimeric GTPases and GTPase-activating proteins in providing the positive charge to facilitate the GTP hydrolysis reaction .
	manualset3
109683	3	403058	5	NULL	NULL	0	NULL	catalytic arginine residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular modelling suggests that this built-in arginine mimics the catalytic arginine residues found in trimeric GTPases and GTPase-activating proteins in providing the positive charge to facilitate the GTP hydrolysis reaction .
	manualset3
109684	4	403058	5	NULL	NULL	NULL	NULL	trimeric GTPases	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Molecular modelling suggests that this built-in arginine mimics the catalytic arginine residues found in trimeric GTPases and GTPase-activating proteins in providing the positive charge to facilitate the GTP hydrolysis reaction .
	manualset3
109685	5	403058	5	NULL	NULL	0	NULL	GTPase-activating proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular modelling suggests that this built-in arginine mimics the catalytic arginine residues found in trimeric GTPases and GTPase-activating proteins in providing the positive charge to facilitate the GTP hydrolysis reaction .
	manualset3
109686	6	403058	5	NULL	NULL	0	NULL	positive charge	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular modelling suggests that this built-in arginine mimics the catalytic arginine residues found in trimeric GTPases and GTPase-activating proteins in providing the positive charge to facilitate the GTP hydrolysis reaction .
	manualset3
109687	7	403058	5	NULL	NULL	0	NULL	GTP hydrolysis reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular modelling suggests that this built-in arginine mimics the catalytic arginine residues found in trimeric GTPases and GTPase-activating proteins in providing the positive charge to facilitate the GTP hydrolysis reaction .
	manualset3
109688	1	403059	5	NULL	NULL	0	NULL	Molecular storage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular storage of ozone in a clathrate hydrate formed from an O3 + O2 + CO2 gas mixture .
	manualset3
109689	2	403059	5	NULL	NULL	0	NULL	ozone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular storage of ozone in a clathrate hydrate formed from an O3 + O2 + CO2 gas mixture .
	manualset3
109690	3	403059	5	NULL	NULL	0	NULL	clathrate hydrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular storage of ozone in a clathrate hydrate formed from an O3 + O2 + CO2 gas mixture .
	manualset3
109691	4	403059	5	NULL	NULL	0	NULL	O3 + O2 + CO2 gas mixture	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular storage of ozone in a clathrate hydrate formed from an O3 + O2 + CO2 gas mixture .
	manualset3
109692	1	403060	5	NULL	NULL	0	NULL	Molecular studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular studies performed on minimally invasive material ( plasma , sputum ) from individuals participating in longitudinal or case-control studies have approximately 70 % -90 % sensitivity and specificity to detect lung cancer .
	manualset3
109693	2	403060	5	NULL	NULL	0	NULL	minimally invasive material	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular studies performed on minimally invasive material ( plasma , sputum ) from individuals participating in longitudinal or case-control studies have approximately 70 % -90 % sensitivity and specificity to detect lung cancer .
	manualset3
109694	3	403060	5	NULL	NULL	NULL	NULL	plasma	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Molecular studies performed on minimally invasive material ( plasma , sputum ) from individuals participating in longitudinal or case-control studies have approximately 70 % -90 % sensitivity and specificity to detect lung cancer .
	manualset3
109695	4	403060	5	NULL	NULL	NULL	NULL	sputum	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Molecular studies performed on minimally invasive material ( plasma , sputum ) from individuals participating in longitudinal or case-control studies have approximately 70 % -90 % sensitivity and specificity to detect lung cancer .
	manualset3
109696	5	403060	5	NULL	NULL	0	NULL	individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular studies performed on minimally invasive material ( plasma , sputum ) from individuals participating in longitudinal or case-control studies have approximately 70 % -90 % sensitivity and specificity to detect lung cancer .
	manualset3
109697	6	403060	5	NULL	NULL	0	NULL	longitudinal studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular studies performed on minimally invasive material ( plasma , sputum ) from individuals participating in longitudinal or case-control studies have approximately 70 % -90 % sensitivity and specificity to detect lung cancer .
	manualset3
109698	7	403060	5	NULL	NULL	0	NULL	case-control studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular studies performed on minimally invasive material ( plasma , sputum ) from individuals participating in longitudinal or case-control studies have approximately 70 % -90 % sensitivity and specificity to detect lung cancer .
	manualset3
109699	8	403060	5	NULL	NULL	0	NULL	70 % -90 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular studies performed on minimally invasive material ( plasma , sputum ) from individuals participating in longitudinal or case-control studies have approximately 70 % -90 % sensitivity and specificity to detect lung cancer .
	manualset3
109700	9	403060	5	NULL	NULL	0	NULL	sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular studies performed on minimally invasive material ( plasma , sputum ) from individuals participating in longitudinal or case-control studies have approximately 70 % -90 % sensitivity and specificity to detect lung cancer .
	manualset3
109701	10	403060	5	NULL	NULL	0	NULL	specificity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular studies performed on minimally invasive material ( plasma , sputum ) from individuals participating in longitudinal or case-control studies have approximately 70 % -90 % sensitivity and specificity to detect lung cancer .
	manualset3
109702	11	403060	5	NULL	NULL	0	NULL	lung cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular studies performed on minimally invasive material ( plasma , sputum ) from individuals participating in longitudinal or case-control studies have approximately 70 % -90 % sensitivity and specificity to detect lung cancer .
	manualset3
109703	1	403061	5	NULL	NULL	0	NULL	Molecular weight dependence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular weight dependence of polyethylene glycol penetration across acetone-disrupted permeability barrier .
	manualset3
109704	2	403061	5	NULL	NULL	0	NULL	polyethylene glycol penetration	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular weight dependence of polyethylene glycol penetration across acetone-disrupted permeability barrier .
	manualset3
109705	3	403061	5	NULL	NULL	NULL	NULL	acetone-disrupted permeability barrier	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Molecular weight dependence of polyethylene glycol penetration across acetone-disrupted permeability barrier .
	manualset3
109713	1	403062	5	NULL	NULL	0	NULL	Molecular weight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular weight estimated by sodium dodecylsulfate gel electrophoresis was about 100 000 .
	manualset3
109714	2	403062	5	NULL	NULL	0	NULL	sodium dodecylsulfate gel electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular weight estimated by sodium dodecylsulfate gel electrophoresis was about 100 000 .
	manualset3
109715	1	403063	5	NULL	NULL	0	NULL	Molecular weight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular weight of human hepatocellular carcinoma ( HCC ) - associated antigen-HL2 antigen was detected to be about 50 , 000 dalton by SDS-PAGE and Western blot .
	manualset3
109716	2	403063	5	NULL	NULL	0	NULL	human hepatocellular carcinoma ( HCC ) - associated antigen-HL2 antigen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular weight of human hepatocellular carcinoma ( HCC ) - associated antigen-HL2 antigen was detected to be about 50 , 000 dalton by SDS-PAGE and Western blot .
	manualset3
109717	3	403063	5	NULL	NULL	0	NULL	50 , 000 dalton	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular weight of human hepatocellular carcinoma ( HCC ) - associated antigen-HL2 antigen was detected to be about 50 , 000 dalton by SDS-PAGE and Western blot .
	manualset3
109718	4	403063	5	NULL	NULL	0	NULL	SDS-PAGE	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular weight of human hepatocellular carcinoma ( HCC ) - associated antigen-HL2 antigen was detected to be about 50 , 000 dalton by SDS-PAGE and Western blot .
	manualset3
109719	5	403063	5	NULL	NULL	0	NULL	Western blot	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular weight of human hepatocellular carcinoma ( HCC ) - associated antigen-HL2 antigen was detected to be about 50 , 000 dalton by SDS-PAGE and Western blot .
	manualset3
109720	1	403064	5	NULL	NULL	0	NULL	Molecules 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecules of N - ( 2-iodophenyl ) -3 - nitrobenzamide ( II ) are linked by a combination of N-H ... O and C-H ... O hydrogen bonds and a two-centre iodo ... carbonyl interaction .
	manualset3
109721	2	403064	5	NULL	NULL	0	NULL	N - ( 2-iodophenyl ) -3 - nitrobenzamide ( II )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecules of N - ( 2-iodophenyl ) -3 - nitrobenzamide ( II ) are linked by a combination of N-H ... O and C-H ... O hydrogen bonds and a two-centre iodo ... carbonyl interaction .
	manualset3
109722	3	403064	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecules of N - ( 2-iodophenyl ) -3 - nitrobenzamide ( II ) are linked by a combination of N-H ... O and C-H ... O hydrogen bonds and a two-centre iodo ... carbonyl interaction .
	manualset3
109723	4	403064	5	NULL	NULL	0	NULL	N-H ... O hydrogen bond	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecules of N - ( 2-iodophenyl ) -3 - nitrobenzamide ( II ) are linked by a combination of N-H ... O and C-H ... O hydrogen bonds and a two-centre iodo ... carbonyl interaction .
	manualset3
109724	5	403064	5	NULL	NULL	NULL	NULL	C-H ... O hydrogen bond	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Molecules of N - ( 2-iodophenyl ) -3 - nitrobenzamide ( II ) are linked by a combination of N-H ... O and C-H ... O hydrogen bonds and a two-centre iodo ... carbonyl interaction .
	manualset3
109725	6	403064	5	NULL	NULL	0	NULL	two-centre iodo ... carbonyl interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecules of N - ( 2-iodophenyl ) -3 - nitrobenzamide ( II ) are linked by a combination of N-H ... O and C-H ... O hydrogen bonds and a two-centre iodo ... carbonyl interaction .
	manualset3
109726	1	403065	5	NULL	NULL	0	NULL	Mollaret meningitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mollaret meningitis is characterized by three or more episodes of benign recurrent aseptic meningitis in which symptoms and signs resolve spontaneously within two to five days .
	manualset3
109727	2	403065	5	NULL	NULL	0	NULL	episodes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mollaret meningitis is characterized by three or more episodes of benign recurrent aseptic meningitis in which symptoms and signs resolve spontaneously within two to five days .
	manualset3
109728	3	403065	5	NULL	NULL	NULL	NULL	benign recurrent aseptic meningitis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mollaret meningitis is characterized by three or more episodes of benign recurrent aseptic meningitis in which symptoms and signs resolve spontaneously within two to five days .
	manualset3
109729	4	403065	5	NULL	NULL	0	NULL	symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mollaret meningitis is characterized by three or more episodes of benign recurrent aseptic meningitis in which symptoms and signs resolve spontaneously within two to five days .
	manualset3
109730	5	403065	5	NULL	NULL	0	NULL	signs 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mollaret meningitis is characterized by three or more episodes of benign recurrent aseptic meningitis in which symptoms and signs resolve spontaneously within two to five days .
	manualset3
109731	6	403065	5	NULL	NULL	0	NULL	 two to five days	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Mollaret meningitis is characterized by three or more episodes of benign recurrent aseptic meningitis in which symptoms and signs resolve spontaneously within two to five days .
	manualset3
112976	7	403065	5	NULL	NULL	0	NULL	three or more 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mollaret meningitis is characterized by three or more episodes of benign recurrent aseptic meningitis in which symptoms and signs resolve spontaneously within two to five days .
	manualset3
109732	1	403066	5	NULL	NULL	0	NULL	Momentum balance equation	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Momentum balance equation for nonelectrolytes in models of coupling between chemical reaction and diffusion in membranes .
	manualset3
109733	2	403066	5	NULL	NULL	0	NULL	nonelectrolytes 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Momentum balance equation for nonelectrolytes in models of coupling between chemical reaction and diffusion in membranes .
	manualset3
109734	3	403066	5	NULL	NULL	0	NULL	models 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Momentum balance equation for nonelectrolytes in models of coupling between chemical reaction and diffusion in membranes .
	manualset3
109735	4	403066	5	NULL	NULL	0	NULL	chemical reaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Momentum balance equation for nonelectrolytes in models of coupling between chemical reaction and diffusion in membranes .
	manualset3
109736	5	403066	5	NULL	NULL	0	NULL	diffusion 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Momentum balance equation for nonelectrolytes in models of coupling between chemical reaction and diffusion in membranes .
	manualset3
109737	6	403066	5	NULL	NULL	0	NULL	membranes 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Momentum balance equation for nonelectrolytes in models of coupling between chemical reaction and diffusion in membranes .
	manualset3
109738	1	403067	5	NULL	NULL	0	NULL	Money 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Money may be a contributing factor to the decision to become sterilized in a large majority of cases , but a dominant motive for only a very small minority .
	manualset3
109739	2	403067	5	NULL	NULL	0	NULL	contributing factor	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Money may be a contributing factor to the decision to become sterilized in a large majority of cases , but a dominant motive for only a very small minority .
	manualset3
109740	3	403067	5	NULL	NULL	NULL	NULL	decision 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Money may be a contributing factor to the decision to become sterilized in a large majority of cases , but a dominant motive for only a very small minority .
	manualset3
109741	4	403067	5	NULL	NULL	0	NULL	 large majority 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Money may be a contributing factor to the decision to become sterilized in a large majority of cases , but a dominant motive for only a very small minority .
	manualset3
109742	5	403067	5	NULL	NULL	0	NULL	cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Money may be a contributing factor to the decision to become sterilized in a large majority of cases , but a dominant motive for only a very small minority .
	manualset3
109743	6	403067	5	NULL	NULL	NULL	NULL	dominant motive	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Money may be a contributing factor to the decision to become sterilized in a large majority of cases , but a dominant motive for only a very small minority .
	manualset3
109744	7	403067	5	NULL	NULL	0	NULL	very small minority	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Money may be a contributing factor to the decision to become sterilized in a large majority of cases , but a dominant motive for only a very small minority .
	manualset3
109745	1	403068	5	NULL	NULL	0	NULL	conductivity changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Monitoring of conductivity changes in passive layers by scanning electrochemical microscopy in feedback mode : localization of pitting precursor sites on surfaces of multimetallic phase materials .
	manualset3
109746	2	403068	5	NULL	NULL	0	NULL	passive layers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Monitoring of conductivity changes in passive layers by scanning electrochemical microscopy in feedback mode : localization of pitting precursor sites on surfaces of multimetallic phase materials .
	manualset3
109747	3	403068	5	NULL	NULL	0	NULL	scanning electrochemical microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Monitoring of conductivity changes in passive layers by scanning electrochemical microscopy in feedback mode : localization of pitting precursor sites on surfaces of multimetallic phase materials .
	manualset3
109748	4	403068	5	NULL	NULL	0	NULL	feedback mode	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Monitoring of conductivity changes in passive layers by scanning electrochemical microscopy in feedback mode : localization of pitting precursor sites on surfaces of multimetallic phase materials .
	manualset3
109749	5	403068	5	NULL	NULL	0	NULL	pitting precursor sites	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Monitoring of conductivity changes in passive layers by scanning electrochemical microscopy in feedback mode : localization of pitting precursor sites on surfaces of multimetallic phase materials .
	manualset3
109750	6	403068	5	NULL	NULL	0	NULL	surfaces 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Monitoring of conductivity changes in passive layers by scanning electrochemical microscopy in feedback mode : localization of pitting precursor sites on surfaces of multimetallic phase materials .
	manualset3
109751	7	403068	5	NULL	NULL	0	NULL	multimetallic phase materials	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Monitoring of conductivity changes in passive layers by scanning electrochemical microscopy in feedback mode : localization of pitting precursor sites on surfaces of multimetallic phase materials .
	manualset3
112977	8	403068	5	NULL	NULL	0	NULL	Monitoring 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Monitoring of conductivity changes in passive layers by scanning electrochemical microscopy in feedback mode : localization of pitting precursor sites on surfaces of multimetallic phase materials .
	manualset3
112978	9	403068	5	NULL	NULL	0	NULL	localization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Monitoring of conductivity changes in passive layers by scanning electrochemical microscopy in feedback mode : localization of pitting precursor sites on surfaces of multimetallic phase materials .
	manualset3
109752	1	403069	5	NULL	NULL	0	NULL	case 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of intra-articular snapping hip caused by articular cartilage detachment from the deformed femoral head consequent to Perthes disease .
	manualset3
109753	2	403069	5	NULL	NULL	0	NULL	intra-articular snapping hip	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of intra-articular snapping hip caused by articular cartilage detachment from the deformed femoral head consequent to Perthes disease .
	manualset3
109754	3	403069	5	NULL	NULL	0	NULL	articular cartilage detachment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of intra-articular snapping hip caused by articular cartilage detachment from the deformed femoral head consequent to Perthes disease .
	manualset3
109755	4	403069	5	NULL	NULL	0	NULL	deformed femoral head	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of intra-articular snapping hip caused by articular cartilage detachment from the deformed femoral head consequent to Perthes disease .
	manualset3
109756	5	403069	5	NULL	NULL	0	NULL	Perthes disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of intra-articular snapping hip caused by articular cartilage detachment from the deformed femoral head consequent to Perthes disease .
	manualset3
109757	1	403070	5	NULL	NULL	0	NULL	Monoamine oxidase ( MAO ) inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoamine oxidase ( MAO ) inhibition is a major consequence of smoking and MAO inhibitors , such as tranylcypromine , increase nicotine reinforcement .
	manualset3
109758	2	403070	5	NULL	NULL	0	NULL	major consequence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoamine oxidase ( MAO ) inhibition is a major consequence of smoking and MAO inhibitors , such as tranylcypromine , increase nicotine reinforcement .
	manualset3
109759	3	403070	5	NULL	NULL	0	NULL	smoking 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoamine oxidase ( MAO ) inhibition is a major consequence of smoking and MAO inhibitors , such as tranylcypromine , increase nicotine reinforcement .
	manualset3
109760	4	403070	5	NULL	NULL	0	NULL	MAO inhibitors	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoamine oxidase ( MAO ) inhibition is a major consequence of smoking and MAO inhibitors , such as tranylcypromine , increase nicotine reinforcement .
	manualset3
109761	5	403070	5	NULL	NULL	NULL	NULL	tranylcypromine 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Monoamine oxidase ( MAO ) inhibition is a major consequence of smoking and MAO inhibitors , such as tranylcypromine , increase nicotine reinforcement .
	manualset3
109762	6	403070	5	NULL	NULL	0	NULL	nicotine reinforcement	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoamine oxidase ( MAO ) inhibition is a major consequence of smoking and MAO inhibitors , such as tranylcypromine , increase nicotine reinforcement .
	manualset3
109763	1	403071	5	NULL	NULL	0	NULL	Monoclonal antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibodies against Yersinia pestis lipopolysaccharide detect bacteria cultured at 28 degrees C or 37 degrees C .
	manualset3
109764	2	403071	5	NULL	NULL	0	NULL	Yersinia pestis lipopolysaccharide	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibodies against Yersinia pestis lipopolysaccharide detect bacteria cultured at 28 degrees C or 37 degrees C .
	manualset3
109765	3	403071	5	NULL	NULL	0	NULL	bacteria 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibodies against Yersinia pestis lipopolysaccharide detect bacteria cultured at 28 degrees C or 37 degrees C .
	manualset3
109766	4	403071	5	NULL	NULL	0	NULL	28 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibodies against Yersinia pestis lipopolysaccharide detect bacteria cultured at 28 degrees C or 37 degrees C .
	manualset3
109767	5	403071	5	NULL	NULL	0	NULL	37 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibodies against Yersinia pestis lipopolysaccharide detect bacteria cultured at 28 degrees C or 37 degrees C .
	manualset3
109768	1	403072	5	NULL	NULL	0	NULL	Monoclonal antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibodies in the detection of bone marrow metastases in small cell lung cancer .
	manualset3
109769	2	403072	5	NULL	NULL	0	NULL	detection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibodies in the detection of bone marrow metastases in small cell lung cancer .
	manualset3
109770	3	403072	5	NULL	NULL	0	NULL	bone marrow metastases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibodies in the detection of bone marrow metastases in small cell lung cancer .
	manualset3
109771	4	403072	5	NULL	NULL	0	NULL	small cell lung cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibodies in the detection of bone marrow metastases in small cell lung cancer .
	manualset3
109772	1	403073	5	NULL	NULL	0	NULL	Monoclonal antibody ( ML-30 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibody ( ML-30 ) directed against 65 kDa stress protein of mycobacteria , is shown to identify human cellular protein homologous with the groEL heat shock protein in many prokaryotes .
	manualset3
109773	2	403073	5	NULL	NULL	0	NULL	65 kDa stress protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibody ( ML-30 ) directed against 65 kDa stress protein of mycobacteria , is shown to identify human cellular protein homologous with the groEL heat shock protein in many prokaryotes .
	manualset3
109774	3	403073	5	NULL	NULL	0	NULL	mycobacteria 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibody ( ML-30 ) directed against 65 kDa stress protein of mycobacteria , is shown to identify human cellular protein homologous with the groEL heat shock protein in many prokaryotes .
	manualset3
109775	4	403073	5	NULL	NULL	0	NULL	human cellular protein homologous with the groEL heat shock protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibody ( ML-30 ) directed against 65 kDa stress protein of mycobacteria , is shown to identify human cellular protein homologous with the groEL heat shock protein in many prokaryotes .
	manualset3
109776	5	403073	5	NULL	NULL	0	NULL	prokaryotes 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibody ( ML-30 ) directed against 65 kDa stress protein of mycobacteria , is shown to identify human cellular protein homologous with the groEL heat shock protein in many prokaryotes .
	manualset3
109777	1	403074	5	NULL	NULL	0	NULL	Monoclonal antibody 1D6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibody 1D6 bound to mutant SP-As in which the neck portion of the molecule was deleted or substituted with that of mannose-binding protein A , but 6E3 failed to bind to these mutants .
	manualset3
109778	2	403074	5	NULL	NULL	NULL	NULL	mutant SP-As	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Monoclonal antibody 1D6 bound to mutant SP-As in which the neck portion of the molecule was deleted or substituted with that of mannose-binding protein A , but 6E3 failed to bind to these mutants .
	manualset3
109779	3	403074	5	NULL	NULL	0	NULL	neck portion	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibody 1D6 bound to mutant SP-As in which the neck portion of the molecule was deleted or substituted with that of mannose-binding protein A , but 6E3 failed to bind to these mutants .
	manualset3
109780	4	403074	5	NULL	NULL	0	NULL	molecule 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibody 1D6 bound to mutant SP-As in which the neck portion of the molecule was deleted or substituted with that of mannose-binding protein A , but 6E3 failed to bind to these mutants .
	manualset3
109781	5	403074	5	NULL	NULL	0	NULL	mannose-binding protein A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibody 1D6 bound to mutant SP-As in which the neck portion of the molecule was deleted or substituted with that of mannose-binding protein A , but 6E3 failed to bind to these mutants .
	manualset3
109782	6	403074	5	NULL	NULL	0	NULL	6E3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibody 1D6 bound to mutant SP-As in which the neck portion of the molecule was deleted or substituted with that of mannose-binding protein A , but 6E3 failed to bind to these mutants .
	manualset3
109783	7	403074	5	NULL	NULL	0	NULL	mutants 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibody 1D6 bound to mutant SP-As in which the neck portion of the molecule was deleted or substituted with that of mannose-binding protein A , but 6E3 failed to bind to these mutants .
	manualset3
109784	1	403075	5	NULL	NULL	0	NULL	Monoclonal antibody staining studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibody staining studies identified the cells in the renal interstitium to be a helper/inducer subset of T lymphocytes .
	manualset3
109785	2	403075	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibody staining studies identified the cells in the renal interstitium to be a helper/inducer subset of T lymphocytes .
	manualset3
109786	3	403075	5	NULL	NULL	0	NULL	renal interstitium 	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibody staining studies identified the cells in the renal interstitium to be a helper/inducer subset of T lymphocytes .
	manualset3
109787	4	403075	5	NULL	NULL	0	NULL	helper/inducer subset 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibody staining studies identified the cells in the renal interstitium to be a helper/inducer subset of T lymphocytes .
	manualset3
109788	5	403075	5	NULL	NULL	0	NULL	T lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibody staining studies identified the cells in the renal interstitium to be a helper/inducer subset of T lymphocytes .
	manualset3
110066	1	403076	5	NULL	NULL	0	NULL	Monocyte chemoattractant protein ( MCP ) -1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Monocyte chemoattractant protein ( MCP ) -1 is expressed by astrocytes in diverse inflammatory states and is a key regulator of monocyte recruitment to the central nervous system ( CNS ) .
	manualset3
110067	2	403076	5	NULL	NULL	0	NULL	astrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Monocyte chemoattractant protein ( MCP ) -1 is expressed by astrocytes in diverse inflammatory states and is a key regulator of monocyte recruitment to the central nervous system ( CNS ) .
	manualset3
110068	3	403076	5	NULL	NULL	0	NULL	diverse inflammatory states	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Monocyte chemoattractant protein ( MCP ) -1 is expressed by astrocytes in diverse inflammatory states and is a key regulator of monocyte recruitment to the central nervous system ( CNS ) .
	manualset3
110069	4	403076	5	NULL	NULL	0	NULL	key regulator	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Monocyte chemoattractant protein ( MCP ) -1 is expressed by astrocytes in diverse inflammatory states and is a key regulator of monocyte recruitment to the central nervous system ( CNS ) .
	manualset3
110070	5	403076	5	NULL	NULL	0	NULL	monocyte recruitment	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Monocyte chemoattractant protein ( MCP ) -1 is expressed by astrocytes in diverse inflammatory states and is a key regulator of monocyte recruitment to the central nervous system ( CNS ) .
	manualset3
110071	6	403076	5	NULL	NULL	0	NULL	central nervous system ( CNS )	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Monocyte chemoattractant protein ( MCP ) -1 is expressed by astrocytes in diverse inflammatory states and is a key regulator of monocyte recruitment to the central nervous system ( CNS ) .
	manualset3
110072	1	403077	5	NULL	NULL	0	NULL	Monocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Monocytes from the blood of a 28-year-old patient were differentiated in media with RANKL and CSF-1 .
	manualset3
110073	2	403077	5	NULL	NULL	0	NULL	blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Monocytes from the blood of a 28-year-old patient were differentiated in media with RANKL and CSF-1 .
	manualset3
110074	3	403077	5	NULL	NULL	0	NULL	28-year-old patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Monocytes from the blood of a 28-year-old patient were differentiated in media with RANKL and CSF-1 .
	manualset3
110075	4	403077	5	NULL	NULL	0	NULL	media	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Monocytes from the blood of a 28-year-old patient were differentiated in media with RANKL and CSF-1 .
	manualset3
110076	5	403077	5	NULL	NULL	0	NULL	RANKL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Monocytes from the blood of a 28-year-old patient were differentiated in media with RANKL and CSF-1 .
	manualset3
110077	6	403077	5	NULL	NULL	0	NULL	CSF-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Monocytes from the blood of a 28-year-old patient were differentiated in media with RANKL and CSF-1 .
	manualset3
110078	1	403078	5	NULL	NULL	0	NULL	Monolayers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Monolayers of octadecanethiol ( ODT ) and the peptide-containing alkanethiol 3-mercapto-N-n-pentadecylpropionamide ( 1ATC15 ) were assembled on gold using the two in situ methods and characterized by contact angle goniometry , X-ray photoelectron spectroscopy , polarization modulation infrared reflection absorption spectroscopy , and electrochemical characterization methods to assess how the monolayer properties compare to those of monolayers prepared by traditional methods .
	manualset3
110079	2	403078	5	NULL	NULL	0	NULL	octadecanethiol ( ODT )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Monolayers of octadecanethiol ( ODT ) and the peptide-containing alkanethiol 3-mercapto-N-n-pentadecylpropionamide ( 1ATC15 ) were assembled on gold using the two in situ methods and characterized by contact angle goniometry , X-ray photoelectron spectroscopy , polarization modulation infrared reflection absorption spectroscopy , and electrochemical characterization methods to assess how the monolayer properties compare to those of monolayers prepared by traditional methods .
	manualset3
110080	3	403078	5	NULL	NULL	0	NULL	alkanethiol 3-mercapto-N-n-pentadecylpropionamide ( 1ATC15 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Monolayers of octadecanethiol ( ODT ) and the peptide-containing alkanethiol 3-mercapto-N-n-pentadecylpropionamide ( 1ATC15 ) were assembled on gold using the two in situ methods and characterized by contact angle goniometry , X-ray photoelectron spectroscopy , polarization modulation infrared reflection absorption spectroscopy , and electrochemical characterization methods to assess how the monolayer properties compare to those of monolayers prepared by traditional methods .
	manualset3
110081	4	403078	5	NULL	NULL	0	NULL	gold	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Monolayers of octadecanethiol ( ODT ) and the peptide-containing alkanethiol 3-mercapto-N-n-pentadecylpropionamide ( 1ATC15 ) were assembled on gold using the two in situ methods and characterized by contact angle goniometry , X-ray photoelectron spectroscopy , polarization modulation infrared reflection absorption spectroscopy , and electrochemical characterization methods to assess how the monolayer properties compare to those of monolayers prepared by traditional methods .
	manualset3
110082	5	403078	5	NULL	NULL	0	NULL	in situ methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Monolayers of octadecanethiol ( ODT ) and the peptide-containing alkanethiol 3-mercapto-N-n-pentadecylpropionamide ( 1ATC15 ) were assembled on gold using the two in situ methods and characterized by contact angle goniometry , X-ray photoelectron spectroscopy , polarization modulation infrared reflection absorption spectroscopy , and electrochemical characterization methods to assess how the monolayer properties compare to those of monolayers prepared by traditional methods .
	manualset3
110083	6	403078	5	NULL	NULL	0	NULL	contact angle goniometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Monolayers of octadecanethiol ( ODT ) and the peptide-containing alkanethiol 3-mercapto-N-n-pentadecylpropionamide ( 1ATC15 ) were assembled on gold using the two in situ methods and characterized by contact angle goniometry , X-ray photoelectron spectroscopy , polarization modulation infrared reflection absorption spectroscopy , and electrochemical characterization methods to assess how the monolayer properties compare to those of monolayers prepared by traditional methods .
	manualset3
110084	7	403078	5	NULL	NULL	0	NULL	X-ray photoelectron spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Monolayers of octadecanethiol ( ODT ) and the peptide-containing alkanethiol 3-mercapto-N-n-pentadecylpropionamide ( 1ATC15 ) were assembled on gold using the two in situ methods and characterized by contact angle goniometry , X-ray photoelectron spectroscopy , polarization modulation infrared reflection absorption spectroscopy , and electrochemical characterization methods to assess how the monolayer properties compare to those of monolayers prepared by traditional methods .
	manualset3
110085	8	403078	5	NULL	NULL	0	NULL	polarization modulation infrared reflection absorption spectroscopy 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Monolayers of octadecanethiol ( ODT ) and the peptide-containing alkanethiol 3-mercapto-N-n-pentadecylpropionamide ( 1ATC15 ) were assembled on gold using the two in situ methods and characterized by contact angle goniometry , X-ray photoelectron spectroscopy , polarization modulation infrared reflection absorption spectroscopy , and electrochemical characterization methods to assess how the monolayer properties compare to those of monolayers prepared by traditional methods .
	manualset3
110086	9	403078	5	NULL	NULL	0	NULL	electrochemical characterization methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Monolayers of octadecanethiol ( ODT ) and the peptide-containing alkanethiol 3-mercapto-N-n-pentadecylpropionamide ( 1ATC15 ) were assembled on gold using the two in situ methods and characterized by contact angle goniometry , X-ray photoelectron spectroscopy , polarization modulation infrared reflection absorption spectroscopy , and electrochemical characterization methods to assess how the monolayer properties compare to those of monolayers prepared by traditional methods .
	manualset3
110087	10	403078	5	NULL	NULL	0	NULL	monolayer properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Monolayers of octadecanethiol ( ODT ) and the peptide-containing alkanethiol 3-mercapto-N-n-pentadecylpropionamide ( 1ATC15 ) were assembled on gold using the two in situ methods and characterized by contact angle goniometry , X-ray photoelectron spectroscopy , polarization modulation infrared reflection absorption spectroscopy , and electrochemical characterization methods to assess how the monolayer properties compare to those of monolayers prepared by traditional methods .
	manualset3
110088	11	403078	5	NULL	NULL	0	NULL	monolayers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Monolayers of octadecanethiol ( ODT ) and the peptide-containing alkanethiol 3-mercapto-N-n-pentadecylpropionamide ( 1ATC15 ) were assembled on gold using the two in situ methods and characterized by contact angle goniometry , X-ray photoelectron spectroscopy , polarization modulation infrared reflection absorption spectroscopy , and electrochemical characterization methods to assess how the monolayer properties compare to those of monolayers prepared by traditional methods .
	manualset3
110089	12	403078	5	NULL	NULL	0	NULL	traditional methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Monolayers of octadecanethiol ( ODT ) and the peptide-containing alkanethiol 3-mercapto-N-n-pentadecylpropionamide ( 1ATC15 ) were assembled on gold using the two in situ methods and characterized by contact angle goniometry , X-ray photoelectron spectroscopy , polarization modulation infrared reflection absorption spectroscopy , and electrochemical characterization methods to assess how the monolayer properties compare to those of monolayers prepared by traditional methods .
	manualset3
110090	1	403079	5	NULL	NULL	0	NULL	Monomelic amyotrophy ( MA )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Monomelic amyotrophy ( MA ) is a variant of motor neuron disease ( MND ) , characterized by muscle weakness and atrophy restricted to one limb .
	manualset3
110091	2	403079	5	NULL	NULL	0	NULL	variant	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Monomelic amyotrophy ( MA ) is a variant of motor neuron disease ( MND ) , characterized by muscle weakness and atrophy restricted to one limb .
	manualset3
110092	3	403079	5	NULL	NULL	0	NULL	motor neuron disease ( MND )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Monomelic amyotrophy ( MA ) is a variant of motor neuron disease ( MND ) , characterized by muscle weakness and atrophy restricted to one limb .
	manualset3
110093	4	403079	5	NULL	NULL	0	NULL	muscle weakness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Monomelic amyotrophy ( MA ) is a variant of motor neuron disease ( MND ) , characterized by muscle weakness and atrophy restricted to one limb .
	manualset3
110094	5	403079	5	NULL	NULL	0	NULL	atrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Monomelic amyotrophy ( MA ) is a variant of motor neuron disease ( MND ) , characterized by muscle weakness and atrophy restricted to one limb .
	manualset3
110095	6	403079	5	NULL	NULL	0	NULL	limb	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Monomelic amyotrophy ( MA ) is a variant of motor neuron disease ( MND ) , characterized by muscle weakness and atrophy restricted to one limb .
	manualset3
110096	1	403080	5	NULL	NULL	0	NULL	Monomorphic ventricular tachycardias	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Monomorphic ventricular tachycardias with sudden onset are characterized by preceding shortening of RR intervals , slower cycle length , and less worsening of ejection fraction .
	manualset3
110097	2	403080	5	NULL	NULL	0	NULL	sudden onset 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Monomorphic ventricular tachycardias with sudden onset are characterized by preceding shortening of RR intervals , slower cycle length , and less worsening of ejection fraction .
	manualset3
110098	3	403080	5	NULL	NULL	0	NULL	preceding shortening of RR intervals	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Monomorphic ventricular tachycardias with sudden onset are characterized by preceding shortening of RR intervals , slower cycle length , and less worsening of ejection fraction .
	manualset3
110099	4	403080	5	NULL	NULL	0	NULL	slower cycle length	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Monomorphic ventricular tachycardias with sudden onset are characterized by preceding shortening of RR intervals , slower cycle length , and less worsening of ejection fraction .
	manualset3
110100	5	403080	5	NULL	NULL	0	NULL	less worsening of ejection fraction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Monomorphic ventricular tachycardias with sudden onset are characterized by preceding shortening of RR intervals , slower cycle length , and less worsening of ejection fraction .
	manualset3
110101	1	403081	5	NULL	NULL	0	NULL	ON -center amacrine cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Monostratified sustained ON - and OFF-center amacrine and ganglion cells rigidly obeyed the border of ON and OFF sublaminae .
	manualset3
110102	2	403081	5	NULL	NULL	0	NULL	OFF-center amacrine cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Monostratified sustained ON - and OFF-center amacrine and ganglion cells rigidly obeyed the border of ON and OFF sublaminae .
	manualset3
110103	3	403081	5	NULL	NULL	0	NULL	ganglion cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Monostratified sustained ON - and OFF-center amacrine and ganglion cells rigidly obeyed the border of ON and OFF sublaminae .
	manualset3
110104	4	403081	5	NULL	NULL	0	NULL	ON sublaminae	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Monostratified sustained ON - and OFF-center amacrine and ganglion cells rigidly obeyed the border of ON and OFF sublaminae .
	manualset3
110105	5	403081	5	NULL	NULL	0	NULL	OFF sublaminae	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Monostratified sustained ON - and OFF-center amacrine and ganglion cells rigidly obeyed the border of ON and OFF sublaminae .
	manualset3
110106	1	403082	5	NULL	NULL	0	NULL	weight loss	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Monthly as well as cumulative weight loss was directly related to the number of days in which food records were kept .
	manualset3
110107	2	403082	5	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Monthly as well as cumulative weight loss was directly related to the number of days in which food records were kept .
	manualset3
110108	3	403082	5	NULL	NULL	0	NULL	days	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Monthly as well as cumulative weight loss was directly related to the number of days in which food records were kept .
	manualset3
110109	4	403082	5	NULL	NULL	0	NULL	food records	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Monthly as well as cumulative weight loss was directly related to the number of days in which food records were kept .
	manualset3
110110	1	403083	5	NULL	NULL	0	NULL	Montmorillonite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Montmorillonite appears to inhibit dechlorination by either inactivating Fe ( II ) by ion exchange or by physically blocking active sites on cement hydration products .
	manualset3
110111	2	403083	5	NULL	NULL	0	NULL	dechlorination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Montmorillonite appears to inhibit dechlorination by either inactivating Fe ( II ) by ion exchange or by physically blocking active sites on cement hydration products .
	manualset3
110112	3	403083	5	NULL	NULL	0	NULL	Fe ( II )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Montmorillonite appears to inhibit dechlorination by either inactivating Fe ( II ) by ion exchange or by physically blocking active sites on cement hydration products .
	manualset3
110113	4	403083	5	NULL	NULL	0	NULL	ion exchange	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Montmorillonite appears to inhibit dechlorination by either inactivating Fe ( II ) by ion exchange or by physically blocking active sites on cement hydration products .
	manualset3
110114	5	403083	5	NULL	NULL	0	NULL	active sites	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Montmorillonite appears to inhibit dechlorination by either inactivating Fe ( II ) by ion exchange or by physically blocking active sites on cement hydration products .
	manualset3
110115	6	403083	5	NULL	NULL	0	NULL	cement hydration products	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Montmorillonite appears to inhibit dechlorination by either inactivating Fe ( II ) by ion exchange or by physically blocking active sites on cement hydration products .
	manualset3
110116	1	403084	5	NULL	NULL	0	NULL	methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	More-rapid methods are available but are very expensive for routine use under program conditions in countries with high levels of tuberculosis endemicity .
	manualset3
110117	2	403084	5	NULL	NULL	0	NULL	routine use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More-rapid methods are available but are very expensive for routine use under program conditions in countries with high levels of tuberculosis endemicity .
	manualset3
110118	3	403084	5	NULL	NULL	0	NULL	program conditions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More-rapid methods are available but are very expensive for routine use under program conditions in countries with high levels of tuberculosis endemicity .
	manualset3
110119	4	403084	5	NULL	NULL	0	NULL	countries	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	More-rapid methods are available but are very expensive for routine use under program conditions in countries with high levels of tuberculosis endemicity .
	manualset3
110120	5	403084	5	NULL	NULL	0	NULL	high levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	More-rapid methods are available but are very expensive for routine use under program conditions in countries with high levels of tuberculosis endemicity .
	manualset3
110121	6	403084	5	NULL	NULL	0	NULL	tuberculosis endemicity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More-rapid methods are available but are very expensive for routine use under program conditions in countries with high levels of tuberculosis endemicity .
	manualset3
110122	1	403085	5	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	More men than women presented with the obsession of need for symmetry .
	manualset3
110123	2	403085	5	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	More men than women presented with the obsession of need for symmetry .
	manualset3
110124	3	403085	5	NULL	NULL	0	NULL	obsession	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	More men than women presented with the obsession of need for symmetry .
	manualset3
110125	4	403085	5	NULL	NULL	0	NULL	need	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More men than women presented with the obsession of need for symmetry .
	manualset3
110126	5	403085	5	NULL	NULL	0	NULL	symmetry	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	More men than women presented with the obsession of need for symmetry .
	manualset3
110131	1	403086	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	More patients in the PGE2 group had a change in Bishop score of ) or = 3 ( 62 % vs. 40 % ; P = 0.002 ) , a Bishop score ) or = 6 after 12 h ( 46 % vs. 34 % ; P = 0.11 ) , and vaginal delivery within 12 h ( 6.5 % vs. 1 % ; P = 0.055 ) .
	manualset3
110132	2	403086	5	NULL	NULL	0	NULL	PGE2 group 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	More patients in the PGE2 group had a change in Bishop score of ) or = 3 ( 62 % vs. 40 % ; P = 0.002 ) , a Bishop score ) or = 6 after 12 h ( 46 % vs. 34 % ; P = 0.11 ) , and vaginal delivery within 12 h ( 6.5 % vs. 1 % ; P = 0.055 ) .
	manualset3
110133	3	403086	5	NULL	NULL	0	NULL	change 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More patients in the PGE2 group had a change in Bishop score of ) or = 3 ( 62 % vs. 40 % ; P = 0.002 ) , a Bishop score ) or = 6 after 12 h ( 46 % vs. 34 % ; P = 0.11 ) , and vaginal delivery within 12 h ( 6.5 % vs. 1 % ; P = 0.055 ) .
	manualset3
110134	4	403086	5	NULL	NULL	NULL	NULL	Bishop score	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	More patients in the PGE2 group had a change in Bishop score of ) or = 3 ( 62 % vs. 40 % ; P = 0.002 ) , a Bishop score ) or = 6 after 12 h ( 46 % vs. 34 % ; P = 0.11 ) , and vaginal delivery within 12 h ( 6.5 % vs. 1 % ; P = 0.055 ) .
	manualset3
110135	5	403086	5	NULL	NULL	0	NULL	3 ( 62 % vs. 40 % ; P = 0.002 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	More patients in the PGE2 group had a change in Bishop score of ) or = 3 ( 62 % vs. 40 % ; P = 0.002 ) , a Bishop score ) or = 6 after 12 h ( 46 % vs. 34 % ; P = 0.11 ) , and vaginal delivery within 12 h ( 6.5 % vs. 1 % ; P = 0.055 ) .
	manualset3
110136	6	403086	5	NULL	NULL	0	NULL	Bishop score	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	More patients in the PGE2 group had a change in Bishop score of ) or = 3 ( 62 % vs. 40 % ; P = 0.002 ) , a Bishop score ) or = 6 after 12 h ( 46 % vs. 34 % ; P = 0.11 ) , and vaginal delivery within 12 h ( 6.5 % vs. 1 % ; P = 0.055 ) .
	manualset3
110137	7	403086	5	NULL	NULL	0	NULL	6 after 12 h ( 46 % vs. 34 % ; P = 0.11 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	More patients in the PGE2 group had a change in Bishop score of ) or = 3 ( 62 % vs. 40 % ; P = 0.002 ) , a Bishop score ) or = 6 after 12 h ( 46 % vs. 34 % ; P = 0.11 ) , and vaginal delivery within 12 h ( 6.5 % vs. 1 % ; P = 0.055 ) .
	manualset3
110138	8	403086	5	NULL	NULL	0	NULL	vaginal delivery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	More patients in the PGE2 group had a change in Bishop score of ) or = 3 ( 62 % vs. 40 % ; P = 0.002 ) , a Bishop score ) or = 6 after 12 h ( 46 % vs. 34 % ; P = 0.11 ) , and vaginal delivery within 12 h ( 6.5 % vs. 1 % ; P = 0.055 ) .
	manualset3
110139	9	403086	5	NULL	NULL	0	NULL	12 h ( 6.5 % vs. 1 % ; P = 0.055 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	More patients in the PGE2 group had a change in Bishop score of ) or = 3 ( 62 % vs. 40 % ; P = 0.002 ) , a Bishop score ) or = 6 after 12 h ( 46 % vs. 34 % ; P = 0.11 ) , and vaginal delivery within 12 h ( 6.5 % vs. 1 % ; P = 0.055 ) .
	manualset3
110140	1	403087	5	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	More studies in Venezuela are recommended , in order to increase our knowledge on the relationship between socioeconomic levels , hemostatic markers and the occurrence of coronary heart disease .
	manualset3
110141	2	403087	5	NULL	NULL	0	NULL	Venezuela 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	More studies in Venezuela are recommended , in order to increase our knowledge on the relationship between socioeconomic levels , hemostatic markers and the occurrence of coronary heart disease .
	manualset3
110142	3	403087	5	NULL	NULL	0	NULL	knowledge 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	More studies in Venezuela are recommended , in order to increase our knowledge on the relationship between socioeconomic levels , hemostatic markers and the occurrence of coronary heart disease .
	manualset3
110143	4	403087	5	NULL	NULL	0	NULL	relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	More studies in Venezuela are recommended , in order to increase our knowledge on the relationship between socioeconomic levels , hemostatic markers and the occurrence of coronary heart disease .
	manualset3
110144	5	403087	5	NULL	NULL	0	NULL	socioeconomic levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	More studies in Venezuela are recommended , in order to increase our knowledge on the relationship between socioeconomic levels , hemostatic markers and the occurrence of coronary heart disease .
	manualset3
110150	6	403087	5	NULL	NULL	0	NULL	hemostatic markers	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	More studies in Venezuela are recommended , in order to increase our knowledge on the relationship between socioeconomic levels , hemostatic markers and the occurrence of coronary heart disease .
	manualset3
110151	7	403087	5	NULL	NULL	0	NULL	occurrence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More studies in Venezuela are recommended , in order to increase our knowledge on the relationship between socioeconomic levels , hemostatic markers and the occurrence of coronary heart disease .
	manualset3
110152	8	403087	5	NULL	NULL	0	NULL	coronary heart disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	More studies in Venezuela are recommended , in order to increase our knowledge on the relationship between socioeconomic levels , hemostatic markers and the occurrence of coronary heart disease .
	manualset3
110153	1	403088	5	NULL	NULL	NULL	NULL	 AIDS organizations	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	More than 30 prominent AIDS organizations issued a consensus statement on the development of protease inhibitors and human growth hormone .
	manualset3
110154	2	403088	5	NULL	NULL	0	NULL	consensus statement 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 30 prominent AIDS organizations issued a consensus statement on the development of protease inhibitors and human growth hormone .
	manualset3
110155	3	403088	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 30 prominent AIDS organizations issued a consensus statement on the development of protease inhibitors and human growth hormone .
	manualset3
110156	4	403088	5	NULL	NULL	0	NULL	protease inhibitors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 30 prominent AIDS organizations issued a consensus statement on the development of protease inhibitors and human growth hormone .
	manualset3
110157	5	403088	5	NULL	NULL	0	NULL	 human growth hormone 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 30 prominent AIDS organizations issued a consensus statement on the development of protease inhibitors and human growth hormone .
	manualset3
110158	6	403088	5	NULL	NULL	0	NULL	30	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 30 prominent AIDS organizations issued a consensus statement on the development of protease inhibitors and human growth hormone .
	manualset3
110159	1	403089	5	NULL	NULL	0	NULL	160	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 160 homologs were tested for effects on antigen presentation by the murine MHC class II alleles : A ( d ) , Ak , E ( d ) , or Ek .
	manualset3
110160	2	403089	5	NULL	NULL	0	NULL	homologs 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 160 homologs were tested for effects on antigen presentation by the murine MHC class II alleles : A ( d ) , Ak , E ( d ) , or Ek .
	manualset3
110161	3	403089	5	NULL	NULL	0	NULL	antigen presentation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 160 homologs were tested for effects on antigen presentation by the murine MHC class II alleles : A ( d ) , Ak , E ( d ) , or Ek .
	manualset3
110162	4	403089	5	NULL	NULL	0	NULL	murine MHC class II alleles	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 160 homologs were tested for effects on antigen presentation by the murine MHC class II alleles : A ( d ) , Ak , E ( d ) , or Ek .
	manualset3
110163	5	403089	5	NULL	NULL	0	NULL	A ( d )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 160 homologs were tested for effects on antigen presentation by the murine MHC class II alleles : A ( d ) , Ak , E ( d ) , or Ek .
	manualset3
110164	6	403089	5	NULL	NULL	0	NULL	Ak	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 160 homologs were tested for effects on antigen presentation by the murine MHC class II alleles : A ( d ) , Ak , E ( d ) , or Ek .
	manualset3
110165	7	403089	5	NULL	NULL	0	NULL	E ( d )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 160 homologs were tested for effects on antigen presentation by the murine MHC class II alleles : A ( d ) , Ak , E ( d ) , or Ek .
	manualset3
110166	8	403089	5	NULL	NULL	0	NULL	Ek	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 160 homologs were tested for effects on antigen presentation by the murine MHC class II alleles : A ( d ) , Ak , E ( d ) , or Ek .
	manualset3
110167	1	403090	5	NULL	NULL	0	NULL	 300	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 300 mutations including insertions-deletions ( indels ) and nucleotide substitutions were found in the intron regions between the NtGA1 and NtGA2 loci , whereas the exon sequences were highly conserved among these and GPA1 .
	manualset3
110168	2	403090	5	NULL	NULL	NULL	NULL	mutations 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	More than 300 mutations including insertions-deletions ( indels ) and nucleotide substitutions were found in the intron regions between the NtGA1 and NtGA2 loci , whereas the exon sequences were highly conserved among these and GPA1 .
	manualset3
110169	3	403090	5	NULL	NULL	0	NULL	insertions-deletions ( indels )	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 300 mutations including insertions-deletions ( indels ) and nucleotide substitutions were found in the intron regions between the NtGA1 and NtGA2 loci , whereas the exon sequences were highly conserved among these and GPA1 .
	manualset3
110170	4	403090	5	NULL	NULL	0	NULL	nucleotide substitutions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 300 mutations including insertions-deletions ( indels ) and nucleotide substitutions were found in the intron regions between the NtGA1 and NtGA2 loci , whereas the exon sequences were highly conserved among these and GPA1 .
	manualset3
110171	5	403090	5	NULL	NULL	0	NULL	intron regions	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 300 mutations including insertions-deletions ( indels ) and nucleotide substitutions were found in the intron regions between the NtGA1 and NtGA2 loci , whereas the exon sequences were highly conserved among these and GPA1 .
	manualset3
110172	6	403090	5	NULL	NULL	NULL	NULL	NtGA1 loci	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	More than 300 mutations including insertions-deletions ( indels ) and nucleotide substitutions were found in the intron regions between the NtGA1 and NtGA2 loci , whereas the exon sequences were highly conserved among these and GPA1 .
	manualset3
110173	7	403090	5	NULL	NULL	0	NULL	NtGA2 loci	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 300 mutations including insertions-deletions ( indels ) and nucleotide substitutions were found in the intron regions between the NtGA1 and NtGA2 loci , whereas the exon sequences were highly conserved among these and GPA1 .
	manualset3
110174	8	403090	5	NULL	NULL	0	NULL	exon sequences 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 300 mutations including insertions-deletions ( indels ) and nucleotide substitutions were found in the intron regions between the NtGA1 and NtGA2 loci , whereas the exon sequences were highly conserved among these and GPA1 .
	manualset3
110175	9	403090	5	NULL	NULL	0	NULL	GPA1 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 300 mutations including insertions-deletions ( indels ) and nucleotide substitutions were found in the intron regions between the NtGA1 and NtGA2 loci , whereas the exon sequences were highly conserved among these and GPA1 .
	manualset3
110176	1	403091	5	NULL	NULL	0	NULL	case 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of parathyroid adenoma causing a spontaneous cervical hematoma is reported .
	manualset3
110177	3	403091	5	NULL	NULL	NULL	NULL	spontaneous cervical hematoma	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A case of parathyroid adenoma causing a spontaneous cervical hematoma is reported .
	manualset3
110178	2	403091	5	NULL	NULL	0	NULL	parathyroid adenoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of parathyroid adenoma causing a spontaneous cervical hematoma is reported .
	manualset3
110179	1	403092	5	NULL	NULL	0	NULL	500 protein spots	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 500 protein spots on each gel were detected by silver staining , of which 150 were excised , digested in-gel with trypsin and characterized by matrix assisted laser desorptioin/ionization-mass spectrometry and tandem electrospray mass spectrometry .
	manualset3
110180	2	403092	5	NULL	NULL	0	NULL	gel 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 500 protein spots on each gel were detected by silver staining , of which 150 were excised , digested in-gel with trypsin and characterized by matrix assisted laser desorptioin/ionization-mass spectrometry and tandem electrospray mass spectrometry .
	manualset3
110181	3	403092	5	NULL	NULL	0	NULL	silver staining	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 500 protein spots on each gel were detected by silver staining , of which 150 were excised , digested in-gel with trypsin and characterized by matrix assisted laser desorptioin/ionization-mass spectrometry and tandem electrospray mass spectrometry .
	manualset3
110182	4	403092	5	NULL	NULL	0	NULL	150	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 500 protein spots on each gel were detected by silver staining , of which 150 were excised , digested in-gel with trypsin and characterized by matrix assisted laser desorptioin/ionization-mass spectrometry and tandem electrospray mass spectrometry .
	manualset3
110183	5	403092	5	NULL	NULL	0	NULL	trypsin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 500 protein spots on each gel were detected by silver staining , of which 150 were excised , digested in-gel with trypsin and characterized by matrix assisted laser desorptioin/ionization-mass spectrometry and tandem electrospray mass spectrometry .
	manualset3
110184	6	403092	5	NULL	NULL	0	NULL	matrix assisted laser desorptioin/ionization-mass spectrometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 500 protein spots on each gel were detected by silver staining , of which 150 were excised , digested in-gel with trypsin and characterized by matrix assisted laser desorptioin/ionization-mass spectrometry and tandem electrospray mass spectrometry .
	manualset3
110185	7	403092	5	NULL	NULL	0	NULL	tandem electrospray mass spectrometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 500 protein spots on each gel were detected by silver staining , of which 150 were excised , digested in-gel with trypsin and characterized by matrix assisted laser desorptioin/ionization-mass spectrometry and tandem electrospray mass spectrometry .
	manualset3
110186	1	403093	5	NULL	NULL	0	NULL	5400 frames	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 5400 frames from MV treatment beam images and 24 CBCT scans were acquired from 12 fractions .
	manualset3
110187	2	403093	5	NULL	NULL	0	NULL	MV treatment beam images	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 5400 frames from MV treatment beam images and 24 CBCT scans were acquired from 12 fractions .
	manualset3
110188	3	403093	5	NULL	NULL	0	NULL	24 CBCT scans	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 5400 frames from MV treatment beam images and 24 CBCT scans were acquired from 12 fractions .
	manualset3
110189	4	403093	5	NULL	NULL	0	NULL	12 fractions	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 5400 frames from MV treatment beam images and 24 CBCT scans were acquired from 12 fractions .
	manualset3
110190	1	403094	5	NULL	NULL	0	NULL	85 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 85 % of all replies asked for more and continuing information related to organ donation and transplantation .
	manualset3
110191	2	403094	5	NULL	NULL	0	NULL	information 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 85 % of all replies asked for more and continuing information related to organ donation and transplantation .
	manualset3
110192	3	403094	5	NULL	NULL	0	NULL	organ donation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 85 % of all replies asked for more and continuing information related to organ donation and transplantation .
	manualset3
110193	4	403094	5	NULL	NULL	0	NULL	transplantation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	More than 85 % of all replies asked for more and continuing information related to organ donation and transplantation .
	manualset3
110194	1	403095	5	NULL	NULL	0	NULL	controls 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	More controls ovulated by 32 h after onset of estrus than were treated cows by 32 h after GnRH , but percentages ( 79 to 94 % ) were similar by 40 h. In multiparous cows , PGF2alpha before Ovsynch increased pregnancy rates , whereas the 2xPG12 protocol produced similar pregnancy rates as Ovsynch across parities .
	manualset3
110195	2	403095	5	NULL	NULL	0	NULL	 32 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	More controls ovulated by 32 h after onset of estrus than were treated cows by 32 h after GnRH , but percentages ( 79 to 94 % ) were similar by 40 h. In multiparous cows , PGF2alpha before Ovsynch increased pregnancy rates , whereas the 2xPG12 protocol produced similar pregnancy rates as Ovsynch across parities .
	manualset3
110196	3	403095	5	NULL	NULL	0	NULL	onset 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More controls ovulated by 32 h after onset of estrus than were treated cows by 32 h after GnRH , but percentages ( 79 to 94 % ) were similar by 40 h. In multiparous cows , PGF2alpha before Ovsynch increased pregnancy rates , whereas the 2xPG12 protocol produced similar pregnancy rates as Ovsynch across parities .
	manualset3
110197	4	403095	5	NULL	NULL	0	NULL	estrus 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	More controls ovulated by 32 h after onset of estrus than were treated cows by 32 h after GnRH , but percentages ( 79 to 94 % ) were similar by 40 h. In multiparous cows , PGF2alpha before Ovsynch increased pregnancy rates , whereas the 2xPG12 protocol produced similar pregnancy rates as Ovsynch across parities .
	manualset3
110198	5	403095	5	NULL	NULL	0	NULL	cows 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	More controls ovulated by 32 h after onset of estrus than were treated cows by 32 h after GnRH , but percentages ( 79 to 94 % ) were similar by 40 h. In multiparous cows , PGF2alpha before Ovsynch increased pregnancy rates , whereas the 2xPG12 protocol produced similar pregnancy rates as Ovsynch across parities .
	manualset3
110199	6	403095	5	NULL	NULL	0	NULL	32 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	More controls ovulated by 32 h after onset of estrus than were treated cows by 32 h after GnRH , but percentages ( 79 to 94 % ) were similar by 40 h. In multiparous cows , PGF2alpha before Ovsynch increased pregnancy rates , whereas the 2xPG12 protocol produced similar pregnancy rates as Ovsynch across parities .
	manualset3
110200	7	403095	5	NULL	NULL	0	NULL	GnRH 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	More controls ovulated by 32 h after onset of estrus than were treated cows by 32 h after GnRH , but percentages ( 79 to 94 % ) were similar by 40 h. In multiparous cows , PGF2alpha before Ovsynch increased pregnancy rates , whereas the 2xPG12 protocol produced similar pregnancy rates as Ovsynch across parities .
	manualset3
110201	8	403095	5	NULL	NULL	0	NULL	percentages 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	More controls ovulated by 32 h after onset of estrus than were treated cows by 32 h after GnRH , but percentages ( 79 to 94 % ) were similar by 40 h. In multiparous cows , PGF2alpha before Ovsynch increased pregnancy rates , whereas the 2xPG12 protocol produced similar pregnancy rates as Ovsynch across parities .
	manualset3
110202	9	403095	5	NULL	NULL	0	NULL	79 to 94 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	More controls ovulated by 32 h after onset of estrus than were treated cows by 32 h after GnRH , but percentages ( 79 to 94 % ) were similar by 40 h. In multiparous cows , PGF2alpha before Ovsynch increased pregnancy rates , whereas the 2xPG12 protocol produced similar pregnancy rates as Ovsynch across parities .
	manualset3
110203	10	403095	5	NULL	NULL	0	NULL	40 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	More controls ovulated by 32 h after onset of estrus than were treated cows by 32 h after GnRH , but percentages ( 79 to 94 % ) were similar by 40 h. In multiparous cows , PGF2alpha before Ovsynch increased pregnancy rates , whereas the 2xPG12 protocol produced similar pregnancy rates as Ovsynch across parities .
	manualset3
110204	11	403095	5	NULL	NULL	0	NULL	multiparous cows	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	More controls ovulated by 32 h after onset of estrus than were treated cows by 32 h after GnRH , but percentages ( 79 to 94 % ) were similar by 40 h. In multiparous cows , PGF2alpha before Ovsynch increased pregnancy rates , whereas the 2xPG12 protocol produced similar pregnancy rates as Ovsynch across parities .
	manualset3
110205	12	403095	5	NULL	NULL	0	NULL	PGF2alpha	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	More controls ovulated by 32 h after onset of estrus than were treated cows by 32 h after GnRH , but percentages ( 79 to 94 % ) were similar by 40 h. In multiparous cows , PGF2alpha before Ovsynch increased pregnancy rates , whereas the 2xPG12 protocol produced similar pregnancy rates as Ovsynch across parities .
	manualset3
110206	13	403095	5	NULL	NULL	0	NULL	Ovsynch 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	More controls ovulated by 32 h after onset of estrus than were treated cows by 32 h after GnRH , but percentages ( 79 to 94 % ) were similar by 40 h. In multiparous cows , PGF2alpha before Ovsynch increased pregnancy rates , whereas the 2xPG12 protocol produced similar pregnancy rates as Ovsynch across parities .
	manualset3
110207	14	403095	5	NULL	NULL	0	NULL	pregnancy rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	More controls ovulated by 32 h after onset of estrus than were treated cows by 32 h after GnRH , but percentages ( 79 to 94 % ) were similar by 40 h. In multiparous cows , PGF2alpha before Ovsynch increased pregnancy rates , whereas the 2xPG12 protocol produced similar pregnancy rates as Ovsynch across parities .
	manualset3
110208	15	403095	5	NULL	NULL	0	NULL	2xPG12 protocol 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	More controls ovulated by 32 h after onset of estrus than were treated cows by 32 h after GnRH , but percentages ( 79 to 94 % ) were similar by 40 h. In multiparous cows , PGF2alpha before Ovsynch increased pregnancy rates , whereas the 2xPG12 protocol produced similar pregnancy rates as Ovsynch across parities .
	manualset3
110209	16	403095	5	NULL	NULL	0	NULL	pregnancy rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	More controls ovulated by 32 h after onset of estrus than were treated cows by 32 h after GnRH , but percentages ( 79 to 94 % ) were similar by 40 h. In multiparous cows , PGF2alpha before Ovsynch increased pregnancy rates , whereas the 2xPG12 protocol produced similar pregnancy rates as Ovsynch across parities .
	manualset3
110210	17	403095	5	NULL	NULL	0	NULL	Ovsynch 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	More controls ovulated by 32 h after onset of estrus than were treated cows by 32 h after GnRH , but percentages ( 79 to 94 % ) were similar by 40 h. In multiparous cows , PGF2alpha before Ovsynch increased pregnancy rates , whereas the 2xPG12 protocol produced similar pregnancy rates as Ovsynch across parities .
	manualset3
110211	18	403095	5	NULL	NULL	0	NULL	parities 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More controls ovulated by 32 h after onset of estrus than were treated cows by 32 h after GnRH , but percentages ( 79 to 94 % ) were similar by 40 h. In multiparous cows , PGF2alpha before Ovsynch increased pregnancy rates , whereas the 2xPG12 protocol produced similar pregnancy rates as Ovsynch across parities .
	manualset3
110212	1	403096	5	NULL	NULL	0	NULL	lymphocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	More lymphocytes were recruited to the site of tumor inoculated by 4T1-ITAC and more than 80 % of these T cells expressed the ITAC receptor , CXCR3 .
	manualset3
110213	2	403096	5	NULL	NULL	0	NULL	site 	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	More lymphocytes were recruited to the site of tumor inoculated by 4T1-ITAC and more than 80 % of these T cells expressed the ITAC receptor , CXCR3 .
	manualset3
110214	3	403096	5	NULL	NULL	0	NULL	tumor 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	More lymphocytes were recruited to the site of tumor inoculated by 4T1-ITAC and more than 80 % of these T cells expressed the ITAC receptor , CXCR3 .
	manualset3
110215	4	403096	5	NULL	NULL	0	NULL	4T1-ITAC 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	More lymphocytes were recruited to the site of tumor inoculated by 4T1-ITAC and more than 80 % of these T cells expressed the ITAC receptor , CXCR3 .
	manualset3
110216	5	403096	5	NULL	NULL	0	NULL	80 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	More lymphocytes were recruited to the site of tumor inoculated by 4T1-ITAC and more than 80 % of these T cells expressed the ITAC receptor , CXCR3 .
	manualset3
110217	6	403096	5	NULL	NULL	0	NULL	T cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	More lymphocytes were recruited to the site of tumor inoculated by 4T1-ITAC and more than 80 % of these T cells expressed the ITAC receptor , CXCR3 .
	manualset3
110218	7	403096	5	NULL	NULL	0	NULL	ITAC receptor , CXCR3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	More lymphocytes were recruited to the site of tumor inoculated by 4T1-ITAC and more than 80 % of these T cells expressed the ITAC receptor , CXCR3 .
	manualset3
110219	1	403097	5	NULL	NULL	0	NULL	mucositis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	More mucositis was seen in arm A. There were four toxic deaths secondary to neutropenia and infection ( one from arm A and three from arm B ) and three other deaths ( two from arm A and one from arm B ) that were possibly drug-related .
	manualset3
110220	2	403097	5	NULL	NULL	0	NULL	arm A	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	More mucositis was seen in arm A. There were four toxic deaths secondary to neutropenia and infection ( one from arm A and three from arm B ) and three other deaths ( two from arm A and one from arm B ) that were possibly drug-related .
	manualset3
110221	3	403097	5	NULL	NULL	NULL	NULL	four toxic deaths	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	More mucositis was seen in arm A. There were four toxic deaths secondary to neutropenia and infection ( one from arm A and three from arm B ) and three other deaths ( two from arm A and one from arm B ) that were possibly drug-related .
	manualset3
110222	4	403097	5	NULL	NULL	0	NULL	neutropenia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	More mucositis was seen in arm A. There were four toxic deaths secondary to neutropenia and infection ( one from arm A and three from arm B ) and three other deaths ( two from arm A and one from arm B ) that were possibly drug-related .
	manualset3
110223	5	403097	5	NULL	NULL	0	NULL	infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	More mucositis was seen in arm A. There were four toxic deaths secondary to neutropenia and infection ( one from arm A and three from arm B ) and three other deaths ( two from arm A and one from arm B ) that were possibly drug-related .
	manualset3
110224	6	403097	5	NULL	NULL	0	NULL	one 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	More mucositis was seen in arm A. There were four toxic deaths secondary to neutropenia and infection ( one from arm A and three from arm B ) and three other deaths ( two from arm A and one from arm B ) that were possibly drug-related .
	manualset3
110225	7	403097	5	NULL	NULL	0	NULL	arm A	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	More mucositis was seen in arm A. There were four toxic deaths secondary to neutropenia and infection ( one from arm A and three from arm B ) and three other deaths ( two from arm A and one from arm B ) that were possibly drug-related .
	manualset3
110226	8	403097	5	NULL	NULL	0	NULL	three 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	More mucositis was seen in arm A. There were four toxic deaths secondary to neutropenia and infection ( one from arm A and three from arm B ) and three other deaths ( two from arm A and one from arm B ) that were possibly drug-related .
	manualset3
110227	9	403097	5	NULL	NULL	0	NULL	arm B	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	More mucositis was seen in arm A. There were four toxic deaths secondary to neutropenia and infection ( one from arm A and three from arm B ) and three other deaths ( two from arm A and one from arm B ) that were possibly drug-related .
	manualset3
110228	10	403097	5	NULL	NULL	0	NULL	three 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	More mucositis was seen in arm A. There were four toxic deaths secondary to neutropenia and infection ( one from arm A and three from arm B ) and three other deaths ( two from arm A and one from arm B ) that were possibly drug-related .
	manualset3
110229	11	403097	5	NULL	NULL	0	NULL	deaths 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	More mucositis was seen in arm A. There were four toxic deaths secondary to neutropenia and infection ( one from arm A and three from arm B ) and three other deaths ( two from arm A and one from arm B ) that were possibly drug-related .
	manualset3
110230	12	403097	5	NULL	NULL	0	NULL	two	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	More mucositis was seen in arm A. There were four toxic deaths secondary to neutropenia and infection ( one from arm A and three from arm B ) and three other deaths ( two from arm A and one from arm B ) that were possibly drug-related .
	manualset3
110232	13	403097	5	NULL	NULL	0	NULL	arm A	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	More mucositis was seen in arm A. There were four toxic deaths secondary to neutropenia and infection ( one from arm A and three from arm B ) and three other deaths ( two from arm A and one from arm B ) that were possibly drug-related .
	manualset3
110233	14	403097	5	NULL	NULL	0	NULL	one	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	More mucositis was seen in arm A. There were four toxic deaths secondary to neutropenia and infection ( one from arm A and three from arm B ) and three other deaths ( two from arm A and one from arm B ) that were possibly drug-related .
	manualset3
110234	15	403097	5	NULL	NULL	0	NULL	arm B	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	More mucositis was seen in arm A. There were four toxic deaths secondary to neutropenia and infection ( one from arm A and three from arm B ) and three other deaths ( two from arm A and one from arm B ) that were possibly drug-related .
	manualset3
110236	1	403098	5	NULL	NULL	0	NULL	neurons 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	More neurons were also obtained when tenuigenin was added in the differentiation medium .
	manualset3
110237	2	403098	5	NULL	NULL	0	NULL	tenuigenin	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	More neurons were also obtained when tenuigenin was added in the differentiation medium .
	manualset3
110238	3	403098	5	NULL	NULL	0	NULL	differentiation medium	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	More neurons were also obtained when tenuigenin was added in the differentiation medium .
	manualset3
110239	1	403099	5	NULL	NULL	0	NULL	research 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	More research is needed in the pediatric population to determine the recommended dietary allowance of vitamin D. A new definition of vitamin D deficiency that would make use of normal serum concentrations of 25-hydroxyvitamin D3 in a given population is needed .
	manualset3
110240	2	403099	5	NULL	NULL	0	NULL	pediatric population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	More research is needed in the pediatric population to determine the recommended dietary allowance of vitamin D. A new definition of vitamin D deficiency that would make use of normal serum concentrations of 25-hydroxyvitamin D3 in a given population is needed .
	manualset3
110241	3	403099	5	NULL	NULL	0	NULL	dietary allowance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More research is needed in the pediatric population to determine the recommended dietary allowance of vitamin D. A new definition of vitamin D deficiency that would make use of normal serum concentrations of 25-hydroxyvitamin D3 in a given population is needed .
	manualset3
110242	4	403099	5	NULL	NULL	0	NULL	vitamin D	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	More research is needed in the pediatric population to determine the recommended dietary allowance of vitamin D. A new definition of vitamin D deficiency that would make use of normal serum concentrations of 25-hydroxyvitamin D3 in a given population is needed .
	manualset3
110243	5	403099	5	NULL	NULL	0	NULL	definition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More research is needed in the pediatric population to determine the recommended dietary allowance of vitamin D. A new definition of vitamin D deficiency that would make use of normal serum concentrations of 25-hydroxyvitamin D3 in a given population is needed .
	manualset3
110244	6	403099	5	NULL	NULL	0	NULL	vitamin D deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	More research is needed in the pediatric population to determine the recommended dietary allowance of vitamin D. A new definition of vitamin D deficiency that would make use of normal serum concentrations of 25-hydroxyvitamin D3 in a given population is needed .
	manualset3
110245	7	403099	5	NULL	NULL	0	NULL	use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More research is needed in the pediatric population to determine the recommended dietary allowance of vitamin D. A new definition of vitamin D deficiency that would make use of normal serum concentrations of 25-hydroxyvitamin D3 in a given population is needed .
	manualset3
110246	8	403099	5	NULL	NULL	0	NULL	normal serum concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	More research is needed in the pediatric population to determine the recommended dietary allowance of vitamin D. A new definition of vitamin D deficiency that would make use of normal serum concentrations of 25-hydroxyvitamin D3 in a given population is needed .
	manualset3
110247	9	403099	5	NULL	NULL	0	NULL	25-hydroxyvitamin D3	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	More research is needed in the pediatric population to determine the recommended dietary allowance of vitamin D. A new definition of vitamin D deficiency that would make use of normal serum concentrations of 25-hydroxyvitamin D3 in a given population is needed .
	manualset3
110248	10	403099	5	NULL	NULL	0	NULL	population 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	More research is needed in the pediatric population to determine the recommended dietary allowance of vitamin D. A new definition of vitamin D deficiency that would make use of normal serum concentrations of 25-hydroxyvitamin D3 in a given population is needed .
	manualset3
110249	1	403100	5	NULL	NULL	0	NULL	case 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of simultaneous occurrence of lichen planus ( LP ) and hepatitis C in the same patient is presented .
	manualset3
110250	2	403100	5	NULL	NULL	0	NULL	 simultaneous occurrence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of simultaneous occurrence of lichen planus ( LP ) and hepatitis C in the same patient is presented .
	manualset3
110251	3	403100	5	NULL	NULL	0	NULL	lichen planus ( LP )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of simultaneous occurrence of lichen planus ( LP ) and hepatitis C in the same patient is presented .
	manualset3
110252	4	403100	5	NULL	NULL	0	NULL	hepatitis C	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of simultaneous occurrence of lichen planus ( LP ) and hepatitis C in the same patient is presented .
	manualset3
110253	5	403100	5	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of simultaneous occurrence of lichen planus ( LP ) and hepatitis C in the same patient is presented .
	manualset3
110254	1	403101	5	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	More studies , with larger sample size , and longer duration will be worthwhile to assess the effect of MCT oil on childhood diarrhea .
	manualset3
110255	2	403101	5	NULL	NULL	0	NULL	larger sample size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	More studies , with larger sample size , and longer duration will be worthwhile to assess the effect of MCT oil on childhood diarrhea .
	manualset3
110256	3	403101	5	NULL	NULL	0	NULL	longer duration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	More studies , with larger sample size , and longer duration will be worthwhile to assess the effect of MCT oil on childhood diarrhea .
	manualset3
110257	4	403101	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More studies , with larger sample size , and longer duration will be worthwhile to assess the effect of MCT oil on childhood diarrhea .
	manualset3
110258	5	403101	5	NULL	NULL	0	NULL	MCT oil	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	More studies , with larger sample size , and longer duration will be worthwhile to assess the effect of MCT oil on childhood diarrhea .
	manualset3
110259	6	403101	5	NULL	NULL	0	NULL	childhood diarrhea	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	More studies , with larger sample size , and longer duration will be worthwhile to assess the effect of MCT oil on childhood diarrhea .
	manualset3
110295	1	403102	5	NULL	NULL	0	NULL	half 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	More than half of TIA patients with symptoms lasting more than 60 min have DWI lesions .
	manualset3
110296	2	403102	5	NULL	NULL	0	NULL	TIA patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	More than half of TIA patients with symptoms lasting more than 60 min have DWI lesions .
	manualset3
110297	3	403102	5	NULL	NULL	0	NULL	symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	More than half of TIA patients with symptoms lasting more than 60 min have DWI lesions .
	manualset3
110298	4	403102	5	NULL	NULL	0	NULL	60 min	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	More than half of TIA patients with symptoms lasting more than 60 min have DWI lesions .
	manualset3
110299	5	403102	5	NULL	NULL	0	NULL	DWI lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	More than half of TIA patients with symptoms lasting more than 60 min have DWI lesions .
	manualset3
110300	1	403103	5	NULL	NULL	0	NULL	half 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	More than half of the cation-pi pairs involve arginine residues , about one-third asparagine or glutamine residues that only carry a partial charge , and one-seventh lysine residues .
	manualset3
110301	2	403103	5	NULL	NULL	0	NULL	cation-pi pairs	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	More than half of the cation-pi pairs involve arginine residues , about one-third asparagine or glutamine residues that only carry a partial charge , and one-seventh lysine residues .
	manualset3
110302	3	403103	5	NULL	NULL	0	NULL	arginine residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	More than half of the cation-pi pairs involve arginine residues , about one-third asparagine or glutamine residues that only carry a partial charge , and one-seventh lysine residues .
	manualset3
110303	4	403103	5	NULL	NULL	0	NULL	one-third	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	More than half of the cation-pi pairs involve arginine residues , about one-third asparagine or glutamine residues that only carry a partial charge , and one-seventh lysine residues .
	manualset3
110304	5	403103	5	NULL	NULL	0	NULL	asparagine 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	More than half of the cation-pi pairs involve arginine residues , about one-third asparagine or glutamine residues that only carry a partial charge , and one-seventh lysine residues .
	manualset3
110305	6	403103	5	NULL	NULL	0	NULL	glutamine residues 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	More than half of the cation-pi pairs involve arginine residues , about one-third asparagine or glutamine residues that only carry a partial charge , and one-seventh lysine residues .
	manualset3
110306	7	403103	5	NULL	NULL	0	NULL	partial charge	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	More than half of the cation-pi pairs involve arginine residues , about one-third asparagine or glutamine residues that only carry a partial charge , and one-seventh lysine residues .
	manualset3
110307	8	403103	5	NULL	NULL	0	NULL	one-seventh 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	More than half of the cation-pi pairs involve arginine residues , about one-third asparagine or glutamine residues that only carry a partial charge , and one-seventh lysine residues .
	manualset3
110308	8	403103	5	NULL	NULL	0	NULL	one-seventh 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	More than half of the cation-pi pairs involve arginine residues , about one-third asparagine or glutamine residues that only carry a partial charge , and one-seventh lysine residues .
	manualset3
110309	9	403103	5	NULL	NULL	0	NULL	lysine residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	More than half of the cation-pi pairs involve arginine residues , about one-third asparagine or glutamine residues that only carry a partial charge , and one-seventh lysine residues .
	manualset3
110310	1	403104	5	NULL	NULL	0	NULL	half 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	More than half of these escapes were found in the initial screening round ( 94 of 168 ) .
	manualset3
110311	2	403104	5	NULL	NULL	0	NULL	escapes 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	More than half of these escapes were found in the initial screening round ( 94 of 168 ) .
	manualset3
110312	3	403104	5	NULL	NULL	0	NULL	initial screening round	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	More than half of these escapes were found in the initial screening round ( 94 of 168 ) .
	manualset3
110313	3	403104	5	NULL	NULL	0	NULL	initial screening round	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	More than half of these escapes were found in the initial screening round ( 94 of 168 ) .
	manualset3
110314	4	403104	5	NULL	NULL	0	NULL	94 of 168	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	More than half of these escapes were found in the initial screening round ( 94 of 168 ) .
	manualset3
110315	1	403105	5	NULL	NULL	0	NULL	complex mechanisms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More complex mechanisms are frequent , especially in the case of immobilized enzymes , and most important is the effect of catalytic modulators ( substrates and products ) on enzyme stability under operation conditions .
	manualset3
110316	2	403105	5	NULL	NULL	0	NULL	case 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	More complex mechanisms are frequent , especially in the case of immobilized enzymes , and most important is the effect of catalytic modulators ( substrates and products ) on enzyme stability under operation conditions .
	manualset3
110317	3	403105	5	NULL	NULL	0	NULL	immobilized enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	More complex mechanisms are frequent , especially in the case of immobilized enzymes , and most important is the effect of catalytic modulators ( substrates and products ) on enzyme stability under operation conditions .
	manualset3
110318	4	403105	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More complex mechanisms are frequent , especially in the case of immobilized enzymes , and most important is the effect of catalytic modulators ( substrates and products ) on enzyme stability under operation conditions .
	manualset3
110319	5	403105	5	NULL	NULL	0	NULL	catalytic modulators	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	More complex mechanisms are frequent , especially in the case of immobilized enzymes , and most important is the effect of catalytic modulators ( substrates and products ) on enzyme stability under operation conditions .
	manualset3
110320	6	403105	5	NULL	NULL	0	NULL	substrates 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	More complex mechanisms are frequent , especially in the case of immobilized enzymes , and most important is the effect of catalytic modulators ( substrates and products ) on enzyme stability under operation conditions .
	manualset3
110321	7	403105	5	NULL	NULL	0	NULL	products 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	More complex mechanisms are frequent , especially in the case of immobilized enzymes , and most important is the effect of catalytic modulators ( substrates and products ) on enzyme stability under operation conditions .
	manualset3
110322	8	403105	5	NULL	NULL	0	NULL	enzyme stability 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	More complex mechanisms are frequent , especially in the case of immobilized enzymes , and most important is the effect of catalytic modulators ( substrates and products ) on enzyme stability under operation conditions .
	manualset3
110323	9	403105	5	NULL	NULL	0	NULL	operation conditions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More complex mechanisms are frequent , especially in the case of immobilized enzymes , and most important is the effect of catalytic modulators ( substrates and products ) on enzyme stability under operation conditions .
	manualset3
110324	1	403106	5	NULL	NULL	0	NULL	lead exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More commonly , significant lead exposure in children occurs in towns that mine , process or transport lead .
	manualset3
110325	2	403106	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	More commonly , significant lead exposure in children occurs in towns that mine , process or transport lead .
	manualset3
110326	3	403106	5	NULL	NULL	0	NULL	towns 	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	More commonly , significant lead exposure in children occurs in towns that mine , process or transport lead .
	manualset3
110331	4	403106	5	NULL	NULL	NULL	NULL	lead 	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	More commonly , significant lead exposure in children occurs in towns that mine , process or transport lead .
	manualset3
110333	1	403107	5	NULL	NULL	0	NULL	message 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	More important , the message catalyzed or sustained changes in the routines of ordinary women , general practitioners , surgeons , and pathologists , which led to the perception that the campaign against cancer was working .
	manualset3
110334	2	403107	5	NULL	NULL	0	NULL	changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More important , the message catalyzed or sustained changes in the routines of ordinary women , general practitioners , surgeons , and pathologists , which led to the perception that the campaign against cancer was working .
	manualset3
110335	3	403107	5	NULL	NULL	0	NULL	routines 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More important , the message catalyzed or sustained changes in the routines of ordinary women , general practitioners , surgeons , and pathologists , which led to the perception that the campaign against cancer was working .
	manualset3
110336	4	403107	5	NULL	NULL	0	NULL	ordinary women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	More important , the message catalyzed or sustained changes in the routines of ordinary women , general practitioners , surgeons , and pathologists , which led to the perception that the campaign against cancer was working .
	manualset3
110337	5	403107	5	NULL	NULL	0	NULL	general practitioners	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	More important , the message catalyzed or sustained changes in the routines of ordinary women , general practitioners , surgeons , and pathologists , which led to the perception that the campaign against cancer was working .
	manualset3
110338	6	403107	5	NULL	NULL	0	NULL	surgeons 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	More important , the message catalyzed or sustained changes in the routines of ordinary women , general practitioners , surgeons , and pathologists , which led to the perception that the campaign against cancer was working .
	manualset3
110339	7	403107	5	NULL	NULL	0	NULL	pathologists 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	More important , the message catalyzed or sustained changes in the routines of ordinary women , general practitioners , surgeons , and pathologists , which led to the perception that the campaign against cancer was working .
	manualset3
110340	8	403107	5	NULL	NULL	0	NULL	perception 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	More important , the message catalyzed or sustained changes in the routines of ordinary women , general practitioners , surgeons , and pathologists , which led to the perception that the campaign against cancer was working .
	manualset3
110342	9	403107	5	NULL	NULL	0	NULL	campaign 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More important , the message catalyzed or sustained changes in the routines of ordinary women , general practitioners , surgeons , and pathologists , which led to the perception that the campaign against cancer was working .
	manualset3
110343	10	403107	5	NULL	NULL	0	NULL	cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	More important , the message catalyzed or sustained changes in the routines of ordinary women , general practitioners , surgeons , and pathologists , which led to the perception that the campaign against cancer was working .
	manualset3
110345	1	403108	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	More importantly , patients with TIM-3-positive tumor cells had a significantly shorter survival time than those with TIM-3-negative tumors .
	manualset3
110346	2	403108	5	NULL	NULL	0	NULL	TIM-3-positive tumor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	More importantly , patients with TIM-3-positive tumor cells had a significantly shorter survival time than those with TIM-3-negative tumors .
	manualset3
110347	2	403108	5	NULL	NULL	0	NULL	TIM-3-positive tumor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	More importantly , patients with TIM-3-positive tumor cells had a significantly shorter survival time than those with TIM-3-negative tumors .
	manualset3
110348	3	403108	5	NULL	NULL	0	NULL	shorter survival time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	More importantly , patients with TIM-3-positive tumor cells had a significantly shorter survival time than those with TIM-3-negative tumors .
	manualset3
110349	4	403108	5	NULL	NULL	0	NULL	TIM-3-negative tumors	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	More importantly , patients with TIM-3-positive tumor cells had a significantly shorter survival time than those with TIM-3-negative tumors .
	manualset3
110350	1	403109	5	NULL	NULL	0	NULL	weak NH-stretching fundamental transition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More importantly , the weak NH-stretching fundamental transition has a pronounced intensity increase upon complexation .
	manualset3
110351	2	403109	5	NULL	NULL	0	NULL	intensity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More importantly , the weak NH-stretching fundamental transition has a pronounced intensity increase upon complexation .
	manualset3
110352	3	403109	5	NULL	NULL	0	NULL	complexation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More importantly , the weak NH-stretching fundamental transition has a pronounced intensity increase upon complexation .
	manualset3
110353	1	403110	5	NULL	NULL	0	NULL	left activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More left than right activity in Brodmann area 45 ( dorso-lateral prefrontal cortex ) and bilateral activity in Brodmann area 44 ( premotor cortex ) exhibited transient hemodynamic responses that did not show any relation to subsequent memory performance .
	manualset3
110355	2	403110	5	NULL	NULL	0	NULL	right activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More left than right activity in Brodmann area 45 ( dorso-lateral prefrontal cortex ) and bilateral activity in Brodmann area 44 ( premotor cortex ) exhibited transient hemodynamic responses that did not show any relation to subsequent memory performance .
	manualset3
110356	3	403110	5	NULL	NULL	0	NULL	Brodmann area 45	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	More left than right activity in Brodmann area 45 ( dorso-lateral prefrontal cortex ) and bilateral activity in Brodmann area 44 ( premotor cortex ) exhibited transient hemodynamic responses that did not show any relation to subsequent memory performance .
	manualset3
110357	4	403110	5	NULL	NULL	0	NULL	dorso-lateral prefrontal cortex	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	More left than right activity in Brodmann area 45 ( dorso-lateral prefrontal cortex ) and bilateral activity in Brodmann area 44 ( premotor cortex ) exhibited transient hemodynamic responses that did not show any relation to subsequent memory performance .
	manualset3
110358	5	403110	5	NULL	NULL	0	NULL	bilateral activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More left than right activity in Brodmann area 45 ( dorso-lateral prefrontal cortex ) and bilateral activity in Brodmann area 44 ( premotor cortex ) exhibited transient hemodynamic responses that did not show any relation to subsequent memory performance .
	manualset3
110360	6	403110	5	NULL	NULL	0	NULL	Brodmann area 44	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	More left than right activity in Brodmann area 45 ( dorso-lateral prefrontal cortex ) and bilateral activity in Brodmann area 44 ( premotor cortex ) exhibited transient hemodynamic responses that did not show any relation to subsequent memory performance .
	manualset3
110362	7	403110	5	NULL	NULL	0	NULL	premotor cortex 	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	More left than right activity in Brodmann area 45 ( dorso-lateral prefrontal cortex ) and bilateral activity in Brodmann area 44 ( premotor cortex ) exhibited transient hemodynamic responses that did not show any relation to subsequent memory performance .
	manualset3
110363	8	403110	5	NULL	NULL	0	NULL	transient hemodynamic responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	More left than right activity in Brodmann area 45 ( dorso-lateral prefrontal cortex ) and bilateral activity in Brodmann area 44 ( premotor cortex ) exhibited transient hemodynamic responses that did not show any relation to subsequent memory performance .
	manualset3
110364	9	403110	5	NULL	NULL	0	NULL	relation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More left than right activity in Brodmann area 45 ( dorso-lateral prefrontal cortex ) and bilateral activity in Brodmann area 44 ( premotor cortex ) exhibited transient hemodynamic responses that did not show any relation to subsequent memory performance .
	manualset3
110366	10	403110	5	NULL	NULL	0	NULL	subsequent memory performance 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	More left than right activity in Brodmann area 45 ( dorso-lateral prefrontal cortex ) and bilateral activity in Brodmann area 44 ( premotor cortex ) exhibited transient hemodynamic responses that did not show any relation to subsequent memory performance .
	manualset3
110369	1	403111	5	NULL	NULL	0	NULL	SH3 domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	More recently , binding of SH3 domains to unusual peptide motifs , folded proteins or lipids has been reported .
	manualset3
110371	2	403111	5	NULL	NULL	0	NULL	unusual peptide motifs	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	More recently , binding of SH3 domains to unusual peptide motifs , folded proteins or lipids has been reported .
	manualset3
110372	3	403111	5	NULL	NULL	0	NULL	folded proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	More recently , binding of SH3 domains to unusual peptide motifs , folded proteins or lipids has been reported .
	manualset3
110373	4	403111	5	NULL	NULL	0	NULL	lipids 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	More recently , binding of SH3 domains to unusual peptide motifs , folded proteins or lipids has been reported .
	manualset3
110374	1	403112	5	NULL	NULL	0	NULL	endothelin-1 ( ET-1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	More recently , endothelin-1 ( ET-1 ) has been found in neural tissues such as spinal cord , brain and peripheral ganglion cells .
	manualset3
110376	2	403112	5	NULL	NULL	0	NULL	neural tissues 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	More recently , endothelin-1 ( ET-1 ) has been found in neural tissues such as spinal cord , brain and peripheral ganglion cells .
	manualset3
110377	3	403112	5	NULL	NULL	0	NULL	spinal cord	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	More recently , endothelin-1 ( ET-1 ) has been found in neural tissues such as spinal cord , brain and peripheral ganglion cells .
	manualset3
110378	4	403112	5	NULL	NULL	0	NULL	brain 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	More recently , endothelin-1 ( ET-1 ) has been found in neural tissues such as spinal cord , brain and peripheral ganglion cells .
	manualset3
110379	5	403112	5	NULL	NULL	0	NULL	peripheral ganglion cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	More recently , endothelin-1 ( ET-1 ) has been found in neural tissues such as spinal cord , brain and peripheral ganglion cells .
	manualset3
110381	1	403113	5	NULL	NULL	0	NULL	post-hoc analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	More recently , post-hoc analysis of the data also showed that repeat hospitalization for ischaemic or bleeding events was decreased with clopidogrel compared with aspirin .
	manualset3
110382	2	403113	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	More recently , post-hoc analysis of the data also showed that repeat hospitalization for ischaemic or bleeding events was decreased with clopidogrel compared with aspirin .
	manualset3
110383	3	403113	5	NULL	NULL	0	NULL	repeat hospitalization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More recently , post-hoc analysis of the data also showed that repeat hospitalization for ischaemic or bleeding events was decreased with clopidogrel compared with aspirin .
	manualset3
110384	4	403113	5	NULL	NULL	0	NULL	ischaemic events	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	More recently , post-hoc analysis of the data also showed that repeat hospitalization for ischaemic or bleeding events was decreased with clopidogrel compared with aspirin .
	manualset3
110385	5	403113	5	NULL	NULL	0	NULL	bleeding events	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	More recently , post-hoc analysis of the data also showed that repeat hospitalization for ischaemic or bleeding events was decreased with clopidogrel compared with aspirin .
	manualset3
110386	6	403113	5	NULL	NULL	0	NULL	clopidogrel 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	More recently , post-hoc analysis of the data also showed that repeat hospitalization for ischaemic or bleeding events was decreased with clopidogrel compared with aspirin .
	manualset3
110387	7	403113	5	NULL	NULL	0	NULL	aspirin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	More recently , post-hoc analysis of the data also showed that repeat hospitalization for ischaemic or bleeding events was decreased with clopidogrel compared with aspirin .
	manualset3
110389	1	403114	5	NULL	NULL	0	NULL	focus 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More recently , the focus has shifted to pinpointing the loci recurrently affected by LOH events across multiple tumors .
	manualset3
110390	2	403114	5	NULL	NULL	0	NULL	loci	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	More recently , the focus has shifted to pinpointing the loci recurrently affected by LOH events across multiple tumors .
	manualset3
110391	3	403114	5	NULL	NULL	0	NULL	LOH events	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	More recently , the focus has shifted to pinpointing the loci recurrently affected by LOH events across multiple tumors .
	manualset3
110392	4	403114	5	NULL	NULL	0	NULL	multiple tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	More recently , the focus has shifted to pinpointing the loci recurrently affected by LOH events across multiple tumors .
	manualset3
110393	1	403115	5	NULL	NULL	0	NULL	question	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More recently , the question of whether early intervention can be targeted at prodromal stage of schizophrenia has called special attention in psychiatry .
	manualset3
110394	2	403115	5	NULL	NULL	0	NULL	early intervention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	More recently , the question of whether early intervention can be targeted at prodromal stage of schizophrenia has called special attention in psychiatry .
	manualset3
110395	3	403115	5	NULL	NULL	0	NULL	prodromal stage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	More recently , the question of whether early intervention can be targeted at prodromal stage of schizophrenia has called special attention in psychiatry .
	manualset3
110396	4	403115	5	NULL	NULL	0	NULL	schizophrenia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	More recently , the question of whether early intervention can be targeted at prodromal stage of schizophrenia has called special attention in psychiatry .
	manualset3
110397	5	403115	5	NULL	NULL	0	NULL	special attention	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	More recently , the question of whether early intervention can be targeted at prodromal stage of schizophrenia has called special attention in psychiatry .
	manualset3
110398	6	403115	5	NULL	NULL	0	NULL	psychiatry	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	More recently , the question of whether early intervention can be targeted at prodromal stage of schizophrenia has called special attention in psychiatry .
	manualset3
110399	1	403116	5	NULL	NULL	0	NULL	case	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of untreated adrenogenital syndrome in a 19 year old patient is described .
	manualset3
110400	2	403116	5	NULL	NULL	0	NULL	untreated adrenogenital syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of untreated adrenogenital syndrome in a 19 year old patient is described .
	manualset3
110401	3	403116	5	NULL	NULL	0	NULL	19 year old patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of untreated adrenogenital syndrome in a 19 year old patient is described .
	manualset3
110402	1	403117	5	NULL	NULL	0	NULL	high degree	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	More significant was the high degree of consistency in the rate of work done by any given lifter in movements which were very similar with respect to joint action , but competitively had very different objectives .
	manualset3
110403	2	403117	5	NULL	NULL	0	NULL	consistency	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More significant was the high degree of consistency in the rate of work done by any given lifter in movements which were very similar with respect to joint action , but competitively had very different objectives .
	manualset3
110404	3	403117	5	NULL	NULL	0	NULL	rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	More significant was the high degree of consistency in the rate of work done by any given lifter in movements which were very similar with respect to joint action , but competitively had very different objectives .
	manualset3
110405	4	403117	5	NULL	NULL	0	NULL	work	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More significant was the high degree of consistency in the rate of work done by any given lifter in movements which were very similar with respect to joint action , but competitively had very different objectives .
	manualset3
110406	5	403117	5	NULL	NULL	0	NULL	lifter	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	More significant was the high degree of consistency in the rate of work done by any given lifter in movements which were very similar with respect to joint action , but competitively had very different objectives .
	manualset3
110407	6	403117	5	NULL	NULL	0	NULL	movements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More significant was the high degree of consistency in the rate of work done by any given lifter in movements which were very similar with respect to joint action , but competitively had very different objectives .
	manualset3
110408	7	403117	5	NULL	NULL	0	NULL	joint action	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More significant was the high degree of consistency in the rate of work done by any given lifter in movements which were very similar with respect to joint action , but competitively had very different objectives .
	manualset3
110409	8	403117	5	NULL	NULL	0	NULL	objectives	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More significant was the high degree of consistency in the rate of work done by any given lifter in movements which were very similar with respect to joint action , but competitively had very different objectives .
	manualset3
110410	1	403118	5	NULL	NULL	0	NULL	displacement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	More significantly , the displacement of cholesterol by ceramide follows a 1 : 1 relation .
	manualset3
110411	2	403118	5	NULL	NULL	0	NULL	cholesterol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	More significantly , the displacement of cholesterol by ceramide follows a 1 : 1 relation .
	manualset3
110412	3	403118	5	NULL	NULL	0	NULL	ceramide	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	More significantly , the displacement of cholesterol by ceramide follows a 1 : 1 relation .
	manualset3
110413	4	403118	5	NULL	NULL	0	NULL	1 : 1 relation	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	More significantly , the displacement of cholesterol by ceramide follows a 1 : 1 relation .
	manualset3
110414	1	403119	5	NULL	NULL	0	NULL	3D mesopore cage adsorbents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , 3D mesopore cage adsorbents are reversible , offering potential for multiple adsorption assays .
	manualset3
110415	2	403119	5	NULL	NULL	0	NULL	potential	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , 3D mesopore cage adsorbents are reversible , offering potential for multiple adsorption assays .
	manualset3
110416	3	403119	5	NULL	NULL	0	NULL	multiple adsorption assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , 3D mesopore cage adsorbents are reversible , offering potential for multiple adsorption assays .
	manualset3
110417	1	403120	5	NULL	NULL	0	NULL	ACAT inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , ACAT inhibition could limit the accumulation of cholesteryl esters in the cytoplasm of macrophages , thus reducing the formation of foam cells .
	manualset3
110418	2	403120	5	NULL	NULL	0	NULL	accumulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , ACAT inhibition could limit the accumulation of cholesteryl esters in the cytoplasm of macrophages , thus reducing the formation of foam cells .
	manualset3
110419	3	403120	5	NULL	NULL	0	NULL	cholesteryl esters	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , ACAT inhibition could limit the accumulation of cholesteryl esters in the cytoplasm of macrophages , thus reducing the formation of foam cells .
	manualset3
110420	4	403120	5	NULL	NULL	0	NULL	cytoplasm	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , ACAT inhibition could limit the accumulation of cholesteryl esters in the cytoplasm of macrophages , thus reducing the formation of foam cells .
	manualset3
110421	5	403120	5	NULL	NULL	0	NULL	macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , ACAT inhibition could limit the accumulation of cholesteryl esters in the cytoplasm of macrophages , thus reducing the formation of foam cells .
	manualset3
110422	6	403120	5	NULL	NULL	0	NULL	formation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , ACAT inhibition could limit the accumulation of cholesteryl esters in the cytoplasm of macrophages , thus reducing the formation of foam cells .
	manualset3
110423	7	403120	5	NULL	NULL	0	NULL	foam cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , ACAT inhibition could limit the accumulation of cholesteryl esters in the cytoplasm of macrophages , thus reducing the formation of foam cells .
	manualset3
110424	1	403121	5	NULL	NULL	0	NULL	DPSCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , DPSCs were found to be able to generate reparative dentin-like tissue on the surface of human dentin in vivo .
	manualset3
110425	2	403121	5	NULL	NULL	0	NULL	reparative dentin-like tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , DPSCs were found to be able to generate reparative dentin-like tissue on the surface of human dentin in vivo .
	manualset3
110426	3	403121	5	NULL	NULL	0	NULL	surface	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , DPSCs were found to be able to generate reparative dentin-like tissue on the surface of human dentin in vivo .
	manualset3
110427	4	403121	5	NULL	NULL	0	NULL	human dentin	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , DPSCs were found to be able to generate reparative dentin-like tissue on the surface of human dentin in vivo .
	manualset3
110428	1	403122	5	NULL	NULL	0	NULL	EA	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , EA at St36 significantly elevated the expression of GAD ( 67 ) mRNA in DG granule cell layer ( GCL ) , but not in the hilus ; neither of the two sham controls showed significant effect on the expression of GAD ( 67 ) mRNA in granule cell layer or hilus .
	manualset3
110429	2	403122	5	NULL	NULL	0	NULL	St36	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , EA at St36 significantly elevated the expression of GAD ( 67 ) mRNA in DG granule cell layer ( GCL ) , but not in the hilus ; neither of the two sham controls showed significant effect on the expression of GAD ( 67 ) mRNA in granule cell layer or hilus .
	manualset3
110430	3	403122	5	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , EA at St36 significantly elevated the expression of GAD ( 67 ) mRNA in DG granule cell layer ( GCL ) , but not in the hilus ; neither of the two sham controls showed significant effect on the expression of GAD ( 67 ) mRNA in granule cell layer or hilus .
	manualset3
110432	4	403122	5	NULL	NULL	0	NULL	GAD ( 67 ) mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , EA at St36 significantly elevated the expression of GAD ( 67 ) mRNA in DG granule cell layer ( GCL ) , but not in the hilus ; neither of the two sham controls showed significant effect on the expression of GAD ( 67 ) mRNA in granule cell layer or hilus .
	manualset3
110433	5	403122	5	NULL	NULL	NULL	NULL	DG granule cell layer ( GCL )	AnatomicalPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Moreover , EA at St36 significantly elevated the expression of GAD ( 67 ) mRNA in DG granule cell layer ( GCL ) , but not in the hilus ; neither of the two sham controls showed significant effect on the expression of GAD ( 67 ) mRNA in granule cell layer or hilus .
	manualset3
110434	6	403122	5	NULL	NULL	0	NULL	hilus	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , EA at St36 significantly elevated the expression of GAD ( 67 ) mRNA in DG granule cell layer ( GCL ) , but not in the hilus ; neither of the two sham controls showed significant effect on the expression of GAD ( 67 ) mRNA in granule cell layer or hilus .
	manualset3
110435	7	403122	5	NULL	NULL	0	NULL	two sham controls	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , EA at St36 significantly elevated the expression of GAD ( 67 ) mRNA in DG granule cell layer ( GCL ) , but not in the hilus ; neither of the two sham controls showed significant effect on the expression of GAD ( 67 ) mRNA in granule cell layer or hilus .
	manualset3
110436	8	403122	5	NULL	NULL	0	NULL	significant effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , EA at St36 significantly elevated the expression of GAD ( 67 ) mRNA in DG granule cell layer ( GCL ) , but not in the hilus ; neither of the two sham controls showed significant effect on the expression of GAD ( 67 ) mRNA in granule cell layer or hilus .
	manualset3
110437	9	403122	5	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , EA at St36 significantly elevated the expression of GAD ( 67 ) mRNA in DG granule cell layer ( GCL ) , but not in the hilus ; neither of the two sham controls showed significant effect on the expression of GAD ( 67 ) mRNA in granule cell layer or hilus .
	manualset3
110438	10	403122	5	NULL	NULL	0	NULL	GAD ( 67 ) mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , EA at St36 significantly elevated the expression of GAD ( 67 ) mRNA in DG granule cell layer ( GCL ) , but not in the hilus ; neither of the two sham controls showed significant effect on the expression of GAD ( 67 ) mRNA in granule cell layer or hilus .
	manualset3
110439	11	403122	5	NULL	NULL	0	NULL	granule cell layer	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , EA at St36 significantly elevated the expression of GAD ( 67 ) mRNA in DG granule cell layer ( GCL ) , but not in the hilus ; neither of the two sham controls showed significant effect on the expression of GAD ( 67 ) mRNA in granule cell layer or hilus .
	manualset3
110440	12	403122	5	NULL	NULL	0	NULL	hilus	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , EA at St36 significantly elevated the expression of GAD ( 67 ) mRNA in DG granule cell layer ( GCL ) , but not in the hilus ; neither of the two sham controls showed significant effect on the expression of GAD ( 67 ) mRNA in granule cell layer or hilus .
	manualset3
110441	1	403123	5	NULL	NULL	NULL	NULL	Heparin administration	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Moreover , Heparin administration significantly inhibited experimental lung metastasis .
	manualset3
110442	2	403123	5	NULL	NULL	0	NULL	experimental lung metastasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , Heparin administration significantly inhibited experimental lung metastasis .
	manualset3
110443	1	403124	5	NULL	NULL	0	NULL	K466/467Q	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , K466/467Q is defective in promoting p53 degradation in living cells .
	manualset3
110444	2	403124	5	NULL	NULL	0	NULL	p53 degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , K466/467Q is defective in promoting p53 degradation in living cells .
	manualset3
110445	3	403124	5	NULL	NULL	0	NULL	living cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , K466/467Q is defective in promoting p53 degradation in living cells .
	manualset3
110446	1	403125	5	NULL	NULL	0	NULL	MAO-B activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , MAO-B activity significantly increased by approximately 100 % at 4 weeks after quitting smoking .
	manualset3
110447	2	403125	5	NULL	NULL	0	NULL	100 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , MAO-B activity significantly increased by approximately 100 % at 4 weeks after quitting smoking .
	manualset3
110448	3	403125	5	NULL	NULL	0	NULL	4 weeks	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , MAO-B activity significantly increased by approximately 100 % at 4 weeks after quitting smoking .
	manualset3
110449	4	403125	5	NULL	NULL	0	NULL	smoking	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , MAO-B activity significantly increased by approximately 100 % at 4 weeks after quitting smoking .
	manualset3
110450	1	403126	5	NULL	NULL	0	NULL	RNA biosynthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , RNA and protein biosynthesis in wild-type CVB3 was significantly inhibited by miR-342-5p .
	manualset3
110451	2	403126	5	NULL	NULL	0	NULL	protein biosynthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , RNA and protein biosynthesis in wild-type CVB3 was significantly inhibited by miR-342-5p .
	manualset3
110452	3	403126	5	NULL	NULL	0	NULL	wild-type CVB3	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , RNA and protein biosynthesis in wild-type CVB3 was significantly inhibited by miR-342-5p .
	manualset3
110453	4	403126	5	NULL	NULL	0	NULL	miR-342-5p	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , RNA and protein biosynthesis in wild-type CVB3 was significantly inhibited by miR-342-5p .
	manualset3
110454	1	403127	5	NULL	NULL	0	NULL	ROS	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , ROS can be generated by radiation ( UV , X-rays ) and pharmacologically , e.g. , by anthracyclins as chemotherapeutic compounds for treatment of a variety of tumors to induce ` stress or aberrant signaling-inducing senescence ' ( STASIS ) .
	manualset3
110455	2	403127	5	NULL	NULL	0	NULL	radiation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , ROS can be generated by radiation ( UV , X-rays ) and pharmacologically , e.g. , by anthracyclins as chemotherapeutic compounds for treatment of a variety of tumors to induce ` stress or aberrant signaling-inducing senescence ' ( STASIS ) .
	manualset3
110456	3	403127	5	NULL	NULL	0	NULL	UV 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , ROS can be generated by radiation ( UV , X-rays ) and pharmacologically , e.g. , by anthracyclins as chemotherapeutic compounds for treatment of a variety of tumors to induce ` stress or aberrant signaling-inducing senescence ' ( STASIS ) .
	manualset3
110457	4	403127	5	NULL	NULL	0	NULL	X-rays	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , ROS can be generated by radiation ( UV , X-rays ) and pharmacologically , e.g. , by anthracyclins as chemotherapeutic compounds for treatment of a variety of tumors to induce ` stress or aberrant signaling-inducing senescence ' ( STASIS ) .
	manualset3
110458	5	403127	5	NULL	NULL	0	NULL	anthracyclins	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , ROS can be generated by radiation ( UV , X-rays ) and pharmacologically , e.g. , by anthracyclins as chemotherapeutic compounds for treatment of a variety of tumors to induce ` stress or aberrant signaling-inducing senescence ' ( STASIS ) .
	manualset3
110459	6	403127	5	NULL	NULL	0	NULL	chemotherapeutic compounds	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , ROS can be generated by radiation ( UV , X-rays ) and pharmacologically , e.g. , by anthracyclins as chemotherapeutic compounds for treatment of a variety of tumors to induce ` stress or aberrant signaling-inducing senescence ' ( STASIS ) .
	manualset3
110460	7	403127	5	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , ROS can be generated by radiation ( UV , X-rays ) and pharmacologically , e.g. , by anthracyclins as chemotherapeutic compounds for treatment of a variety of tumors to induce ` stress or aberrant signaling-inducing senescence ' ( STASIS ) .
	manualset3
110461	8	403127	5	NULL	NULL	0	NULL	variety	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , ROS can be generated by radiation ( UV , X-rays ) and pharmacologically , e.g. , by anthracyclins as chemotherapeutic compounds for treatment of a variety of tumors to induce ` stress or aberrant signaling-inducing senescence ' ( STASIS ) .
	manualset3
110462	9	403127	5	NULL	NULL	0	NULL	tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , ROS can be generated by radiation ( UV , X-rays ) and pharmacologically , e.g. , by anthracyclins as chemotherapeutic compounds for treatment of a variety of tumors to induce ` stress or aberrant signaling-inducing senescence ' ( STASIS ) .
	manualset3
110463	10	403127	5	NULL	NULL	0	NULL	` stress or aberrant signaling-inducing senescence ' ( STASIS )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , ROS can be generated by radiation ( UV , X-rays ) and pharmacologically , e.g. , by anthracyclins as chemotherapeutic compounds for treatment of a variety of tumors to induce ` stress or aberrant signaling-inducing senescence ' ( STASIS ) .
	manualset3
110464	1	403128	5	NULL	NULL	0	NULL	STIM1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , STIM1 and STIM1 ( K684E , K685E ) reciprocally affected receptor-activated WT and mutant TRPC channels .
	manualset3
110465	2	403128	5	NULL	NULL	0	NULL	STIM1 ( K684E , K685E )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , STIM1 and STIM1 ( K684E , K685E ) reciprocally affected receptor-activated WT and mutant TRPC channels .
	manualset3
110466	3	403128	5	NULL	NULL	0	NULL	receptor-activated WT	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , STIM1 and STIM1 ( K684E , K685E ) reciprocally affected receptor-activated WT and mutant TRPC channels .
	manualset3
110467	4	403128	5	NULL	NULL	0	NULL	mutant TRPC channels	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , STIM1 and STIM1 ( K684E , K685E ) reciprocally affected receptor-activated WT and mutant TRPC channels .
	manualset3
110468	1	403129	5	NULL	NULL	0	NULL	TLR signals	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , TLR signals stimulate not only pro-inflammatory cytokines such as IFNs , IL-1 , TNFalpha , and IL-12 but also anti-inflammatory cytokines such as IL-10 and IL-6 IL-12 and IL-10 are cytokines that bridge early innate responses and the ensuing specific immune responses .
	manualset3
110469	2	403129	5	NULL	NULL	0	NULL	pro-inflammatory cytokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , TLR signals stimulate not only pro-inflammatory cytokines such as IFNs , IL-1 , TNFalpha , and IL-12 but also anti-inflammatory cytokines such as IL-10 and IL-6 IL-12 and IL-10 are cytokines that bridge early innate responses and the ensuing specific immune responses .
	manualset3
110470	3	403129	5	NULL	NULL	0	NULL	 IFNs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , TLR signals stimulate not only pro-inflammatory cytokines such as IFNs , IL-1 , TNFalpha , and IL-12 but also anti-inflammatory cytokines such as IL-10 and IL-6 IL-12 and IL-10 are cytokines that bridge early innate responses and the ensuing specific immune responses .
	manualset3
110471	4	403129	5	NULL	NULL	0	NULL	IL-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , TLR signals stimulate not only pro-inflammatory cytokines such as IFNs , IL-1 , TNFalpha , and IL-12 but also anti-inflammatory cytokines such as IL-10 and IL-6 IL-12 and IL-10 are cytokines that bridge early innate responses and the ensuing specific immune responses .
	manualset3
110472	5	403129	5	NULL	NULL	0	NULL	TNFalpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , TLR signals stimulate not only pro-inflammatory cytokines such as IFNs , IL-1 , TNFalpha , and IL-12 but also anti-inflammatory cytokines such as IL-10 and IL-6 IL-12 and IL-10 are cytokines that bridge early innate responses and the ensuing specific immune responses .
	manualset3
110473	6	403129	5	NULL	NULL	0	NULL	IL-12 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , TLR signals stimulate not only pro-inflammatory cytokines such as IFNs , IL-1 , TNFalpha , and IL-12 but also anti-inflammatory cytokines such as IL-10 and IL-6 IL-12 and IL-10 are cytokines that bridge early innate responses and the ensuing specific immune responses .
	manualset3
110474	7	403129	5	NULL	NULL	0	NULL	anti-inflammatory cytokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , TLR signals stimulate not only pro-inflammatory cytokines such as IFNs , IL-1 , TNFalpha , and IL-12 but also anti-inflammatory cytokines such as IL-10 and IL-6 IL-12 and IL-10 are cytokines that bridge early innate responses and the ensuing specific immune responses .
	manualset3
110475	8	403129	5	NULL	NULL	0	NULL	IL-10	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , TLR signals stimulate not only pro-inflammatory cytokines such as IFNs , IL-1 , TNFalpha , and IL-12 but also anti-inflammatory cytokines such as IL-10 and IL-6 IL-12 and IL-10 are cytokines that bridge early innate responses and the ensuing specific immune responses .
	manualset3
110476	9	403129	5	NULL	NULL	NULL	NULL	IL-6	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Moreover , TLR signals stimulate not only pro-inflammatory cytokines such as IFNs , IL-1 , TNFalpha , and IL-12 but also anti-inflammatory cytokines such as IL-10 and IL-6 IL-12 and IL-10 are cytokines that bridge early innate responses and the ensuing specific immune responses .
	manualset3
110477	10	403129	5	NULL	NULL	0	NULL	IL-12	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , TLR signals stimulate not only pro-inflammatory cytokines such as IFNs , IL-1 , TNFalpha , and IL-12 but also anti-inflammatory cytokines such as IL-10 and IL-6 IL-12 and IL-10 are cytokines that bridge early innate responses and the ensuing specific immune responses .
	manualset3
110478	11	403129	5	NULL	NULL	0	NULL	IL-10	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , TLR signals stimulate not only pro-inflammatory cytokines such as IFNs , IL-1 , TNFalpha , and IL-12 but also anti-inflammatory cytokines such as IL-10 and IL-6 IL-12 and IL-10 are cytokines that bridge early innate responses and the ensuing specific immune responses .
	manualset3
110479	12	403129	5	NULL	NULL	0	NULL	cytokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , TLR signals stimulate not only pro-inflammatory cytokines such as IFNs , IL-1 , TNFalpha , and IL-12 but also anti-inflammatory cytokines such as IL-10 and IL-6 IL-12 and IL-10 are cytokines that bridge early innate responses and the ensuing specific immune responses .
	manualset3
110480	13	403129	5	NULL	NULL	0	NULL	early innate responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , TLR signals stimulate not only pro-inflammatory cytokines such as IFNs , IL-1 , TNFalpha , and IL-12 but also anti-inflammatory cytokines such as IL-10 and IL-6 IL-12 and IL-10 are cytokines that bridge early innate responses and the ensuing specific immune responses .
	manualset3
110481	14	403129	5	NULL	NULL	0	NULL	specific immune responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , TLR signals stimulate not only pro-inflammatory cytokines such as IFNs , IL-1 , TNFalpha , and IL-12 but also anti-inflammatory cytokines such as IL-10 and IL-6 IL-12 and IL-10 are cytokines that bridge early innate responses and the ensuing specific immune responses .
	manualset3
110482	1	403130	5	NULL	NULL	0	NULL	high vascular index	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , a high vascular index in neuroblastoma correlates with poor prognosis , suggesting dependence of aggressive tumor growth on active angiogenesis .
	manualset3
110483	2	403130	5	NULL	NULL	0	NULL	neuroblastoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , a high vascular index in neuroblastoma correlates with poor prognosis , suggesting dependence of aggressive tumor growth on active angiogenesis .
	manualset3
110484	3	403130	5	NULL	NULL	0	NULL	poor prognosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , a high vascular index in neuroblastoma correlates with poor prognosis , suggesting dependence of aggressive tumor growth on active angiogenesis .
	manualset3
110485	4	403130	5	NULL	NULL	0	NULL	dependence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , a high vascular index in neuroblastoma correlates with poor prognosis , suggesting dependence of aggressive tumor growth on active angiogenesis .
	manualset3
110486	5	403130	5	NULL	NULL	0	NULL	aggressive tumor growth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , a high vascular index in neuroblastoma correlates with poor prognosis , suggesting dependence of aggressive tumor growth on active angiogenesis .
	manualset3
110487	6	403130	5	NULL	NULL	0	NULL	active angiogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , a high vascular index in neuroblastoma correlates with poor prognosis , suggesting dependence of aggressive tumor growth on active angiogenesis .
	manualset3
110807	1	403131	5	NULL	NULL	0	NULL	miniaturized cell exposure system	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , a miniaturized cell exposure system was validated for further experiments using fewer amounts of hepatocytes and contaminants , and allowing exposure to PAH metabolites .
	manualset3
110808	2	403131	5	NULL	NULL	0	NULL	experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , a miniaturized cell exposure system was validated for further experiments using fewer amounts of hepatocytes and contaminants , and allowing exposure to PAH metabolites .
	manualset3
110809	3	403131	5	NULL	NULL	0	NULL	fewer amounts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , a miniaturized cell exposure system was validated for further experiments using fewer amounts of hepatocytes and contaminants , and allowing exposure to PAH metabolites .
	manualset3
110810	4	403131	5	NULL	NULL	0	NULL	hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , a miniaturized cell exposure system was validated for further experiments using fewer amounts of hepatocytes and contaminants , and allowing exposure to PAH metabolites .
	manualset3
110811	5	403131	5	NULL	NULL	0	NULL	contaminants	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , a miniaturized cell exposure system was validated for further experiments using fewer amounts of hepatocytes and contaminants , and allowing exposure to PAH metabolites .
	manualset3
110812	6	403131	5	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , a miniaturized cell exposure system was validated for further experiments using fewer amounts of hepatocytes and contaminants , and allowing exposure to PAH metabolites .
	manualset3
110813	7	403131	5	NULL	NULL	0	NULL	PAH metabolites	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , a miniaturized cell exposure system was validated for further experiments using fewer amounts of hepatocytes and contaminants , and allowing exposure to PAH metabolites .
	manualset3
110814	1	403132	5	NULL	NULL	0	NULL	phylogenetic tree	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , a phylogenetic tree of scorpion toxins has been constructed , which , together with the worldwide distribution of toxins and the zoogeographic dispersion of the studied genera , offers an insight into the evolution of diverse scorpion toxins .
	manualset3
110815	2	403132	5	NULL	NULL	0	NULL	scorpion toxins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , a phylogenetic tree of scorpion toxins has been constructed , which , together with the worldwide distribution of toxins and the zoogeographic dispersion of the studied genera , offers an insight into the evolution of diverse scorpion toxins .
	manualset3
110816	3	403132	5	NULL	NULL	0	NULL	worldwide distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , a phylogenetic tree of scorpion toxins has been constructed , which , together with the worldwide distribution of toxins and the zoogeographic dispersion of the studied genera , offers an insight into the evolution of diverse scorpion toxins .
	manualset3
110817	4	403132	5	NULL	NULL	0	NULL	toxins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , a phylogenetic tree of scorpion toxins has been constructed , which , together with the worldwide distribution of toxins and the zoogeographic dispersion of the studied genera , offers an insight into the evolution of diverse scorpion toxins .
	manualset3
110818	5	403132	5	NULL	NULL	0	NULL	zoogeographic dispersion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , a phylogenetic tree of scorpion toxins has been constructed , which , together with the worldwide distribution of toxins and the zoogeographic dispersion of the studied genera , offers an insight into the evolution of diverse scorpion toxins .
	manualset3
110819	6	403132	5	NULL	NULL	0	NULL	genera	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , a phylogenetic tree of scorpion toxins has been constructed , which , together with the worldwide distribution of toxins and the zoogeographic dispersion of the studied genera , offers an insight into the evolution of diverse scorpion toxins .
	manualset3
110820	7	403132	5	NULL	NULL	0	NULL	insight	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , a phylogenetic tree of scorpion toxins has been constructed , which , together with the worldwide distribution of toxins and the zoogeographic dispersion of the studied genera , offers an insight into the evolution of diverse scorpion toxins .
	manualset3
110821	8	403132	5	NULL	NULL	0	NULL	evolution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , a phylogenetic tree of scorpion toxins has been constructed , which , together with the worldwide distribution of toxins and the zoogeographic dispersion of the studied genera , offers an insight into the evolution of diverse scorpion toxins .
	manualset3
110822	9	403132	5	NULL	NULL	0	NULL	diverse scorpion toxins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , a phylogenetic tree of scorpion toxins has been constructed , which , together with the worldwide distribution of toxins and the zoogeographic dispersion of the studied genera , offers an insight into the evolution of diverse scorpion toxins .
	manualset3
110823	1	403133	5	NULL	NULL	0	NULL	polydentate ligand	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , as the polydentate ligand is prepared from the same hapten used for the immunogen synthesis , this type of noncompetitive immunoassay appears generally applicable to all small molecules for which antibodies have been obtained .
	manualset3
110824	2	403133	5	NULL	NULL	0	NULL	hapten	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , as the polydentate ligand is prepared from the same hapten used for the immunogen synthesis , this type of noncompetitive immunoassay appears generally applicable to all small molecules for which antibodies have been obtained .
	manualset3
110825	3	403133	5	NULL	NULL	0	NULL	immunogen synthesis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , as the polydentate ligand is prepared from the same hapten used for the immunogen synthesis , this type of noncompetitive immunoassay appears generally applicable to all small molecules for which antibodies have been obtained .
	manualset3
110826	4	403133	5	NULL	NULL	0	NULL	noncompetitive immunoassay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , as the polydentate ligand is prepared from the same hapten used for the immunogen synthesis , this type of noncompetitive immunoassay appears generally applicable to all small molecules for which antibodies have been obtained .
	manualset3
110827	5	403133	5	NULL	NULL	0	NULL	small molecules	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , as the polydentate ligand is prepared from the same hapten used for the immunogen synthesis , this type of noncompetitive immunoassay appears generally applicable to all small molecules for which antibodies have been obtained .
	manualset3
110828	6	403133	5	NULL	NULL	0	NULL	antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , as the polydentate ligand is prepared from the same hapten used for the immunogen synthesis , this type of noncompetitive immunoassay appears generally applicable to all small molecules for which antibodies have been obtained .
	manualset3
110829	1	403134	5	NULL	NULL	0	NULL	biological behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , biological behavior of breast cancer among Japanese females has been recently changing .
	manualset3
110830	2	403134	5	NULL	NULL	0	NULL	breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , biological behavior of breast cancer among Japanese females has been recently changing .
	manualset3
110831	3	403134	5	NULL	NULL	0	NULL	Japanese females	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , biological behavior of breast cancer among Japanese females has been recently changing .
	manualset3
110832	1	403135	5	NULL	NULL	0	NULL	Tyr-protein kinases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , both Tyr-protein kinases exhibit several identical properties , including Km values for band 3 , the random acidic copolymer poly ( Glu , Tyr ) 4 : 1 and angiotensin II , pH dependence , response to Mn2 + and Mg2 + , response to NaCl and 2 , 3-bisphosphoglycerate .
	manualset3
110833	2	403135	5	NULL	NULL	0	NULL	identical properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , both Tyr-protein kinases exhibit several identical properties , including Km values for band 3 , the random acidic copolymer poly ( Glu , Tyr ) 4 : 1 and angiotensin II , pH dependence , response to Mn2 + and Mg2 + , response to NaCl and 2 , 3-bisphosphoglycerate .
	manualset3
110834	3	403135	5	NULL	NULL	0	NULL	Km values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , both Tyr-protein kinases exhibit several identical properties , including Km values for band 3 , the random acidic copolymer poly ( Glu , Tyr ) 4 : 1 and angiotensin II , pH dependence , response to Mn2 + and Mg2 + , response to NaCl and 2 , 3-bisphosphoglycerate .
	manualset3
110835	4	403135	5	NULL	NULL	0	NULL	band 3	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , both Tyr-protein kinases exhibit several identical properties , including Km values for band 3 , the random acidic copolymer poly ( Glu , Tyr ) 4 : 1 and angiotensin II , pH dependence , response to Mn2 + and Mg2 + , response to NaCl and 2 , 3-bisphosphoglycerate .
	manualset3
110836	5	403135	5	NULL	NULL	NULL	NULL	random acidic copolymer poly ( Glu , Tyr ) 4 : 1	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Moreover , both Tyr-protein kinases exhibit several identical properties , including Km values for band 3 , the random acidic copolymer poly ( Glu , Tyr ) 4 : 1 and angiotensin II , pH dependence , response to Mn2 + and Mg2 + , response to NaCl and 2 , 3-bisphosphoglycerate .
	manualset3
110837	6	403135	5	NULL	NULL	0	NULL	angiotensin II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , both Tyr-protein kinases exhibit several identical properties , including Km values for band 3 , the random acidic copolymer poly ( Glu , Tyr ) 4 : 1 and angiotensin II , pH dependence , response to Mn2 + and Mg2 + , response to NaCl and 2 , 3-bisphosphoglycerate .
	manualset3
110838	7	403135	5	NULL	NULL	0	NULL	pH dependence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , both Tyr-protein kinases exhibit several identical properties , including Km values for band 3 , the random acidic copolymer poly ( Glu , Tyr ) 4 : 1 and angiotensin II , pH dependence , response to Mn2 + and Mg2 + , response to NaCl and 2 , 3-bisphosphoglycerate .
	manualset3
110839	8	403135	5	NULL	NULL	NULL	NULL	response to Mn2 +	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Moreover , both Tyr-protein kinases exhibit several identical properties , including Km values for band 3 , the random acidic copolymer poly ( Glu , Tyr ) 4 : 1 and angiotensin II , pH dependence , response to Mn2 + and Mg2 + , response to NaCl and 2 , 3-bisphosphoglycerate .
	manualset3
110840	9	403135	5	NULL	NULL	NULL	NULL	response to Mg2 +	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Moreover , both Tyr-protein kinases exhibit several identical properties , including Km values for band 3 , the random acidic copolymer poly ( Glu , Tyr ) 4 : 1 and angiotensin II , pH dependence , response to Mn2 + and Mg2 + , response to NaCl and 2 , 3-bisphosphoglycerate .
	manualset3
110841	10	403135	5	NULL	NULL	0	NULL	response to NaCl	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , both Tyr-protein kinases exhibit several identical properties , including Km values for band 3 , the random acidic copolymer poly ( Glu , Tyr ) 4 : 1 and angiotensin II , pH dependence , response to Mn2 + and Mg2 + , response to NaCl and 2 , 3-bisphosphoglycerate .
	manualset3
110842	11	403135	5	NULL	NULL	0	NULL	response to 2 , 3-bisphosphoglycerate	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , both Tyr-protein kinases exhibit several identical properties , including Km values for band 3 , the random acidic copolymer poly ( Glu , Tyr ) 4 : 1 and angiotensin II , pH dependence , response to Mn2 + and Mg2 + , response to NaCl and 2 , 3-bisphosphoglycerate .
	manualset3
110843	1	403136	5	NULL	NULL	0	NULL	carbohydrates	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , both carbohydrates significantly increased the intestinal absorption and balance of Ca and Mg , without altering the plasma level of these two minerals .
	manualset3
110844	2	403136	5	NULL	NULL	0	NULL	intestinal absorption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , both carbohydrates significantly increased the intestinal absorption and balance of Ca and Mg , without altering the plasma level of these two minerals .
	manualset3
110845	3	403136	5	NULL	NULL	0	NULL	balance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , both carbohydrates significantly increased the intestinal absorption and balance of Ca and Mg , without altering the plasma level of these two minerals .
	manualset3
110846	4	403136	5	NULL	NULL	0	NULL	Ca	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , both carbohydrates significantly increased the intestinal absorption and balance of Ca and Mg , without altering the plasma level of these two minerals .
	manualset3
110847	5	403136	5	NULL	NULL	0	NULL	Mg	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , both carbohydrates significantly increased the intestinal absorption and balance of Ca and Mg , without altering the plasma level of these two minerals .
	manualset3
110848	6	403136	5	NULL	NULL	0	NULL	plasma level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , both carbohydrates significantly increased the intestinal absorption and balance of Ca and Mg , without altering the plasma level of these two minerals .
	manualset3
110849	7	403136	5	NULL	NULL	0	NULL	minerals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , both carbohydrates significantly increased the intestinal absorption and balance of Ca and Mg , without altering the plasma level of these two minerals .
	manualset3
110850	1	403137	5	NULL	NULL	0	NULL	case report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A case report is presented of the anesthetic management of a parturient with paramyotonia congenita and lupus anticoagulant antibodies .
	manualset3
110851	2	403137	5	NULL	NULL	0	NULL	anesthetic management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A case report is presented of the anesthetic management of a parturient with paramyotonia congenita and lupus anticoagulant antibodies .
	manualset3
110852	3	403137	5	NULL	NULL	0	NULL	parturient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A case report is presented of the anesthetic management of a parturient with paramyotonia congenita and lupus anticoagulant antibodies .
	manualset3
110853	4	403137	5	NULL	NULL	0	NULL	paramyotonia congenita	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A case report is presented of the anesthetic management of a parturient with paramyotonia congenita and lupus anticoagulant antibodies .
	manualset3
110854	5	403137	5	NULL	NULL	0	NULL	lupus anticoagulant antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A case report is presented of the anesthetic management of a parturient with paramyotonia congenita and lupus anticoagulant antibodies .
	manualset3
110855	1	403138	5	NULL	NULL	NULL	NULL	compounds	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Moreover , both compounds have shown to be able to cross the blood-brain barrier and , therefore , they can be considered as potential antidepressants .
	manualset3
110856	2	403138	5	NULL	NULL	0	NULL	blood-brain barrier	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , both compounds have shown to be able to cross the blood-brain barrier and , therefore , they can be considered as potential antidepressants .
	manualset3
110857	3	403138	5	NULL	NULL	0	NULL	potential antidepressants	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , both compounds have shown to be able to cross the blood-brain barrier and , therefore , they can be considered as potential antidepressants .
	manualset3
110858	1	403139	5	NULL	NULL	0	NULL	chorda tympani section	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , chorda tympani section led to decrease in the saliva secretion and the PI value of the patients in the early and late postoperative period .
	manualset3
110859	2	403139	5	NULL	NULL	0	NULL	saliva secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , chorda tympani section led to decrease in the saliva secretion and the PI value of the patients in the early and late postoperative period .
	manualset3
110860	3	403139	5	NULL	NULL	0	NULL	PI value	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , chorda tympani section led to decrease in the saliva secretion and the PI value of the patients in the early and late postoperative period .
	manualset3
110861	4	403139	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , chorda tympani section led to decrease in the saliva secretion and the PI value of the patients in the early and late postoperative period .
	manualset3
110862	5	403139	5	NULL	NULL	0	NULL	early postoperative period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , chorda tympani section led to decrease in the saliva secretion and the PI value of the patients in the early and late postoperative period .
	manualset3
110863	6	403139	5	NULL	NULL	0	NULL	late postoperative period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , chorda tympani section led to decrease in the saliva secretion and the PI value of the patients in the early and late postoperative period .
	manualset3
110864	1	403140	5	NULL	NULL	0	NULL	anti-LFA-1 monoclonal antibody ( mAb )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , co-crosslinking with anti-LFA-1 monoclonal antibody ( mAb ) and suboptimal concentration of anti-CD3 mAb markedly increases tyrosine phosphorylation of FAK in an antibody-concentration and time-dependent manner compared with stimulation through CD3 alone .
	manualset3
110874	2	403140	5	NULL	NULL	0	NULL	suboptimal concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , co-crosslinking with anti-LFA-1 monoclonal antibody ( mAb ) and suboptimal concentration of anti-CD3 mAb markedly increases tyrosine phosphorylation of FAK in an antibody-concentration and time-dependent manner compared with stimulation through CD3 alone .
	manualset3
110875	3	403140	5	NULL	NULL	0	NULL	anti-CD3 mAb	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , co-crosslinking with anti-LFA-1 monoclonal antibody ( mAb ) and suboptimal concentration of anti-CD3 mAb markedly increases tyrosine phosphorylation of FAK in an antibody-concentration and time-dependent manner compared with stimulation through CD3 alone .
	manualset3
110876	4	403140	5	NULL	NULL	0	NULL	tyrosine phosphorylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , co-crosslinking with anti-LFA-1 monoclonal antibody ( mAb ) and suboptimal concentration of anti-CD3 mAb markedly increases tyrosine phosphorylation of FAK in an antibody-concentration and time-dependent manner compared with stimulation through CD3 alone .
	manualset3
110877	5	403140	5	NULL	NULL	0	NULL	FAK 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , co-crosslinking with anti-LFA-1 monoclonal antibody ( mAb ) and suboptimal concentration of anti-CD3 mAb markedly increases tyrosine phosphorylation of FAK in an antibody-concentration and time-dependent manner compared with stimulation through CD3 alone .
	manualset3
110878	6	403140	5	NULL	NULL	0	NULL	antibody-concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , co-crosslinking with anti-LFA-1 monoclonal antibody ( mAb ) and suboptimal concentration of anti-CD3 mAb markedly increases tyrosine phosphorylation of FAK in an antibody-concentration and time-dependent manner compared with stimulation through CD3 alone .
	manualset3
110879	7	403140	5	NULL	NULL	0	NULL	time-dependent manner	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , co-crosslinking with anti-LFA-1 monoclonal antibody ( mAb ) and suboptimal concentration of anti-CD3 mAb markedly increases tyrosine phosphorylation of FAK in an antibody-concentration and time-dependent manner compared with stimulation through CD3 alone .
	manualset3
110880	8	403140	5	NULL	NULL	0	NULL	stimulation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , co-crosslinking with anti-LFA-1 monoclonal antibody ( mAb ) and suboptimal concentration of anti-CD3 mAb markedly increases tyrosine phosphorylation of FAK in an antibody-concentration and time-dependent manner compared with stimulation through CD3 alone .
	manualset3
110881	9	403140	5	NULL	NULL	0	NULL	CD3 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , co-crosslinking with anti-LFA-1 monoclonal antibody ( mAb ) and suboptimal concentration of anti-CD3 mAb markedly increases tyrosine phosphorylation of FAK in an antibody-concentration and time-dependent manner compared with stimulation through CD3 alone .
	manualset3
110882	1	403141	5	NULL	NULL	0	NULL	conversion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , conversion of gliotoxin to its dithiol derivative by addition of reduced dithiothreitol during incubation protected cells from losing oxidase activity .
	manualset3
110883	2	403141	5	NULL	NULL	0	NULL	gliotoxin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , conversion of gliotoxin to its dithiol derivative by addition of reduced dithiothreitol during incubation protected cells from losing oxidase activity .
	manualset3
110884	3	403141	5	NULL	NULL	0	NULL	dithiol derivative	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , conversion of gliotoxin to its dithiol derivative by addition of reduced dithiothreitol during incubation protected cells from losing oxidase activity .
	manualset3
110885	4	403141	5	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , conversion of gliotoxin to its dithiol derivative by addition of reduced dithiothreitol during incubation protected cells from losing oxidase activity .
	manualset3
110886	5	403141	5	NULL	NULL	0	NULL	reduced dithiothreitol 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , conversion of gliotoxin to its dithiol derivative by addition of reduced dithiothreitol during incubation protected cells from losing oxidase activity .
	manualset3
110887	6	403141	5	NULL	NULL	0	NULL	incubation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , conversion of gliotoxin to its dithiol derivative by addition of reduced dithiothreitol during incubation protected cells from losing oxidase activity .
	manualset3
110888	7	403141	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , conversion of gliotoxin to its dithiol derivative by addition of reduced dithiothreitol during incubation protected cells from losing oxidase activity .
	manualset3
122141	8	403141	5	NULL	NULL	0	NULL	oxidase activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , conversion of gliotoxin to its dithiol derivative by addition of reduced dithiothreitol during incubation protected cells from losing oxidase activity .
	manualset3
110889	1	403142	5	NULL	NULL	0	NULL	coronary spasm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , coronary spasm was not induced by the intracoronary injection of ergonovine .
	manualset3
110890	2	403142	5	NULL	NULL	0	NULL	intracoronary injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , coronary spasm was not induced by the intracoronary injection of ergonovine .
	manualset3
110891	3	403142	5	NULL	NULL	0	NULL	ergonovine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , coronary spasm was not induced by the intracoronary injection of ergonovine .
	manualset3
110892	1	403143	5	NULL	NULL	0	NULL	SC5 molecules	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , cross-linking of SC5 molecules inhibited the malignant cell proliferation induced by anti-CD3 mAbs .
	manualset3
110893	2	403143	5	NULL	NULL	0	NULL	malignant cell proliferation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , cross-linking of SC5 molecules inhibited the malignant cell proliferation induced by anti-CD3 mAbs .
	manualset3
110894	3	403143	5	NULL	NULL	0	NULL	anti-CD3 mAbs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , cross-linking of SC5 molecules inhibited the malignant cell proliferation induced by anti-CD3 mAbs .
	manualset3
110895	1	403144	5	NULL	NULL	0	NULL	cyclic AMP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , cyclic AMP has been shown to increase the rate of capillary endothelial pinocytosis and produce brain edema .
	manualset3
110896	2	403144	5	NULL	NULL	0	NULL	rate 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , cyclic AMP has been shown to increase the rate of capillary endothelial pinocytosis and produce brain edema .
	manualset3
110897	3	403144	5	NULL	NULL	0	NULL	capillary endothelial pinocytosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , cyclic AMP has been shown to increase the rate of capillary endothelial pinocytosis and produce brain edema .
	manualset3
110901	4	403144	5	NULL	NULL	0	NULL	brain edema	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , cyclic AMP has been shown to increase the rate of capillary endothelial pinocytosis and produce brain edema .
	manualset3
110902	1	403145	5	NULL	NULL	0	NULL	exogenous LacCer 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , exogenous LacCer recovered the reduced expression of RANK and the phosphorylation of inhibitor of NF-kappa B and extracellular signal-regulated kinase 1/2 after stimulation by RANKL at the same level of cells without D-PDMP treatment .
	manualset3
110903	2	403145	5	NULL	NULL	0	NULL	reduced expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , exogenous LacCer recovered the reduced expression of RANK and the phosphorylation of inhibitor of NF-kappa B and extracellular signal-regulated kinase 1/2 after stimulation by RANKL at the same level of cells without D-PDMP treatment .
	manualset3
110904	3	403145	5	NULL	NULL	0	NULL	RANK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , exogenous LacCer recovered the reduced expression of RANK and the phosphorylation of inhibitor of NF-kappa B and extracellular signal-regulated kinase 1/2 after stimulation by RANKL at the same level of cells without D-PDMP treatment .
	manualset3
110905	4	403145	5	NULL	NULL	0	NULL	phosphorylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , exogenous LacCer recovered the reduced expression of RANK and the phosphorylation of inhibitor of NF-kappa B and extracellular signal-regulated kinase 1/2 after stimulation by RANKL at the same level of cells without D-PDMP treatment .
	manualset3
110906	5	403145	5	NULL	NULL	0	NULL	inhibitor of NF-kappa B 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , exogenous LacCer recovered the reduced expression of RANK and the phosphorylation of inhibitor of NF-kappa B and extracellular signal-regulated kinase 1/2 after stimulation by RANKL at the same level of cells without D-PDMP treatment .
	manualset3
110907	6	403145	5	NULL	NULL	0	NULL	extracellular signal-regulated kinase 1/2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , exogenous LacCer recovered the reduced expression of RANK and the phosphorylation of inhibitor of NF-kappa B and extracellular signal-regulated kinase 1/2 after stimulation by RANKL at the same level of cells without D-PDMP treatment .
	manualset3
110908	7	403145	5	NULL	NULL	0	NULL	stimulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , exogenous LacCer recovered the reduced expression of RANK and the phosphorylation of inhibitor of NF-kappa B and extracellular signal-regulated kinase 1/2 after stimulation by RANKL at the same level of cells without D-PDMP treatment .
	manualset3
110909	8	403145	5	NULL	NULL	0	NULL	RANKL 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , exogenous LacCer recovered the reduced expression of RANK and the phosphorylation of inhibitor of NF-kappa B and extracellular signal-regulated kinase 1/2 after stimulation by RANKL at the same level of cells without D-PDMP treatment .
	manualset3
110910	9	403145	5	NULL	NULL	0	NULL	same level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , exogenous LacCer recovered the reduced expression of RANK and the phosphorylation of inhibitor of NF-kappa B and extracellular signal-regulated kinase 1/2 after stimulation by RANKL at the same level of cells without D-PDMP treatment .
	manualset3
110912	10	403145	5	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , exogenous LacCer recovered the reduced expression of RANK and the phosphorylation of inhibitor of NF-kappa B and extracellular signal-regulated kinase 1/2 after stimulation by RANKL at the same level of cells without D-PDMP treatment .
	manualset3
110913	11	403145	5	NULL	NULL	0	NULL	D-PDMP treatment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , exogenous LacCer recovered the reduced expression of RANK and the phosphorylation of inhibitor of NF-kappa B and extracellular signal-regulated kinase 1/2 after stimulation by RANKL at the same level of cells without D-PDMP treatment .
	manualset3
110914	1	403146	5	NULL	NULL	0	NULL	case report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A case report of a newborn with sepsis due to nontypable H. Influenzae biotype IV is presented .
	manualset3
110916	2	403146	5	NULL	NULL	0	NULL	newborn 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A case report of a newborn with sepsis due to nontypable H. Influenzae biotype IV is presented .
	manualset3
110918	3	403146	5	NULL	NULL	0	NULL	sepsis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A case report of a newborn with sepsis due to nontypable H. Influenzae biotype IV is presented .
	manualset3
110926	4	403146	5	NULL	NULL	0	NULL	nontypable H. Influenzae biotype IV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A case report of a newborn with sepsis due to nontypable H. Influenzae biotype IV is presented .
	manualset3
110927	1	403147	5	NULL	NULL	0	NULL	cell types	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , in both cell types , A-II receptors were coupled to intracellular effectors since A-II : 1 ) stimulated the accumulation of inositol phosphates , although the effects in BAC were higher than in OAC ; 2 ) enhanced the influx and the efflux of 45Ca2 + ; 3 ) increased cytosolic free Ca2 + concentration ( ( Ca2 + ) i ) ; 4 ) potentiated ACTH-induced cAMP production ; and 5 ) induced A-II receptor loss .
	manualset3
110928	2	403147	5	NULL	NULL	0	NULL	A-II receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , in both cell types , A-II receptors were coupled to intracellular effectors since A-II : 1 ) stimulated the accumulation of inositol phosphates , although the effects in BAC were higher than in OAC ; 2 ) enhanced the influx and the efflux of 45Ca2 + ; 3 ) increased cytosolic free Ca2 + concentration ( ( Ca2 + ) i ) ; 4 ) potentiated ACTH-induced cAMP production ; and 5 ) induced A-II receptor loss .
	manualset3
110929	3	403147	5	NULL	NULL	0	NULL	intracellular effectors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , in both cell types , A-II receptors were coupled to intracellular effectors since A-II : 1 ) stimulated the accumulation of inositol phosphates , although the effects in BAC were higher than in OAC ; 2 ) enhanced the influx and the efflux of 45Ca2 + ; 3 ) increased cytosolic free Ca2 + concentration ( ( Ca2 + ) i ) ; 4 ) potentiated ACTH-induced cAMP production ; and 5 ) induced A-II receptor loss .
	manualset3
110933	4	403147	5	NULL	NULL	0	NULL	A-II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , in both cell types , A-II receptors were coupled to intracellular effectors since A-II : 1 ) stimulated the accumulation of inositol phosphates , although the effects in BAC were higher than in OAC ; 2 ) enhanced the influx and the efflux of 45Ca2 + ; 3 ) increased cytosolic free Ca2 + concentration ( ( Ca2 + ) i ) ; 4 ) potentiated ACTH-induced cAMP production ; and 5 ) induced A-II receptor loss .
	manualset3
110934	5	403147	5	NULL	NULL	0	NULL	accumulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , in both cell types , A-II receptors were coupled to intracellular effectors since A-II : 1 ) stimulated the accumulation of inositol phosphates , although the effects in BAC were higher than in OAC ; 2 ) enhanced the influx and the efflux of 45Ca2 + ; 3 ) increased cytosolic free Ca2 + concentration ( ( Ca2 + ) i ) ; 4 ) potentiated ACTH-induced cAMP production ; and 5 ) induced A-II receptor loss .
	manualset3
110936	6	403147	5	NULL	NULL	0	NULL	inositol phosphates	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , in both cell types , A-II receptors were coupled to intracellular effectors since A-II : 1 ) stimulated the accumulation of inositol phosphates , although the effects in BAC were higher than in OAC ; 2 ) enhanced the influx and the efflux of 45Ca2 + ; 3 ) increased cytosolic free Ca2 + concentration ( ( Ca2 + ) i ) ; 4 ) potentiated ACTH-induced cAMP production ; and 5 ) induced A-II receptor loss .
	manualset3
110939	7	403147	5	NULL	NULL	0	NULL	BAC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , in both cell types , A-II receptors were coupled to intracellular effectors since A-II : 1 ) stimulated the accumulation of inositol phosphates , although the effects in BAC were higher than in OAC ; 2 ) enhanced the influx and the efflux of 45Ca2 + ; 3 ) increased cytosolic free Ca2 + concentration ( ( Ca2 + ) i ) ; 4 ) potentiated ACTH-induced cAMP production ; and 5 ) induced A-II receptor loss .
	manualset3
110940	8	403147	5	NULL	NULL	0	NULL	OAC 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , in both cell types , A-II receptors were coupled to intracellular effectors since A-II : 1 ) stimulated the accumulation of inositol phosphates , although the effects in BAC were higher than in OAC ; 2 ) enhanced the influx and the efflux of 45Ca2 + ; 3 ) increased cytosolic free Ca2 + concentration ( ( Ca2 + ) i ) ; 4 ) potentiated ACTH-induced cAMP production ; and 5 ) induced A-II receptor loss .
	manualset3
110941	9	403147	5	NULL	NULL	NULL	NULL	influx	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Moreover , in both cell types , A-II receptors were coupled to intracellular effectors since A-II : 1 ) stimulated the accumulation of inositol phosphates , although the effects in BAC were higher than in OAC ; 2 ) enhanced the influx and the efflux of 45Ca2 + ; 3 ) increased cytosolic free Ca2 + concentration ( ( Ca2 + ) i ) ; 4 ) potentiated ACTH-induced cAMP production ; and 5 ) induced A-II receptor loss .
	manualset3
110943	10	403147	5	NULL	NULL	0	NULL	efflux 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , in both cell types , A-II receptors were coupled to intracellular effectors since A-II : 1 ) stimulated the accumulation of inositol phosphates , although the effects in BAC were higher than in OAC ; 2 ) enhanced the influx and the efflux of 45Ca2 + ; 3 ) increased cytosolic free Ca2 + concentration ( ( Ca2 + ) i ) ; 4 ) potentiated ACTH-induced cAMP production ; and 5 ) induced A-II receptor loss .
	manualset3
110944	11	403147	5	NULL	NULL	0	NULL	45Ca2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , in both cell types , A-II receptors were coupled to intracellular effectors since A-II : 1 ) stimulated the accumulation of inositol phosphates , although the effects in BAC were higher than in OAC ; 2 ) enhanced the influx and the efflux of 45Ca2 + ; 3 ) increased cytosolic free Ca2 + concentration ( ( Ca2 + ) i ) ; 4 ) potentiated ACTH-induced cAMP production ; and 5 ) induced A-II receptor loss .
	manualset3
110945	12	403147	5	NULL	NULL	0	NULL	cytosolic free Ca2 + concentration ( ( Ca2 + ) i )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , in both cell types , A-II receptors were coupled to intracellular effectors since A-II : 1 ) stimulated the accumulation of inositol phosphates , although the effects in BAC were higher than in OAC ; 2 ) enhanced the influx and the efflux of 45Ca2 + ; 3 ) increased cytosolic free Ca2 + concentration ( ( Ca2 + ) i ) ; 4 ) potentiated ACTH-induced cAMP production ; and 5 ) induced A-II receptor loss .
	manualset3
110946	13	403147	5	NULL	NULL	0	NULL	ACTH-induced cAMP production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , in both cell types , A-II receptors were coupled to intracellular effectors since A-II : 1 ) stimulated the accumulation of inositol phosphates , although the effects in BAC were higher than in OAC ; 2 ) enhanced the influx and the efflux of 45Ca2 + ; 3 ) increased cytosolic free Ca2 + concentration ( ( Ca2 + ) i ) ; 4 ) potentiated ACTH-induced cAMP production ; and 5 ) induced A-II receptor loss .
	manualset3
110947	14	403147	5	NULL	NULL	0	NULL	A-II receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , in both cell types , A-II receptors were coupled to intracellular effectors since A-II : 1 ) stimulated the accumulation of inositol phosphates , although the effects in BAC were higher than in OAC ; 2 ) enhanced the influx and the efflux of 45Ca2 + ; 3 ) increased cytosolic free Ca2 + concentration ( ( Ca2 + ) i ) ; 4 ) potentiated ACTH-induced cAMP production ; and 5 ) induced A-II receptor loss .
	manualset3
110948	1	403148	5	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , in the present study , we measured hind limb length as a new endpoint of thyroid axis .
	manualset3
110949	2	403148	5	NULL	NULL	0	NULL	hind limb	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , in the present study , we measured hind limb length as a new endpoint of thyroid axis .
	manualset3
110952	3	403148	5	NULL	NULL	0	NULL	length	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , in the present study , we measured hind limb length as a new endpoint of thyroid axis .
	manualset3
110953	4	403148	5	NULL	NULL	NULL	NULL	new endpoint 	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Moreover , in the present study , we measured hind limb length as a new endpoint of thyroid axis .
	manualset3
110957	5	403148	5	NULL	NULL	0	NULL	thyroid axis	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , in the present study , we measured hind limb length as a new endpoint of thyroid axis .
	manualset3
110961	1	403149	5	NULL	NULL	NULL	NULL	treatment group	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Moreover , in the treatment and prophylaxis groups , bacterial counts of Streptococcus equi subsp .
	manualset3
110962	2	403149	5	NULL	NULL	0	NULL	prophylaxis group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , in the treatment and prophylaxis groups , bacterial counts of Streptococcus equi subsp .
	manualset3
110963	3	403149	5	NULL	NULL	0	NULL	bacterial counts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , in the treatment and prophylaxis groups , bacterial counts of Streptococcus equi subsp .
	manualset3
110964	4	403149	5	NULL	NULL	0	NULL	Streptococcus equi subsp	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , in the treatment and prophylaxis groups , bacterial counts of Streptococcus equi subsp .
	manualset3
110965	1	403150	5	NULL	NULL	0	NULL	transcription activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , increased transcription activity of c-Jun by the JNK activation contributed to the down-regulation of MDR1 , thus indicating a central role of JNK signalling to suppress P-gp level in 5-Aza-treated Caki-1 cells .
	manualset3
110966	2	403150	5	NULL	NULL	0	NULL	c-Jun 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , increased transcription activity of c-Jun by the JNK activation contributed to the down-regulation of MDR1 , thus indicating a central role of JNK signalling to suppress P-gp level in 5-Aza-treated Caki-1 cells .
	manualset3
110967	3	403150	5	NULL	NULL	0	NULL	JNK activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , increased transcription activity of c-Jun by the JNK activation contributed to the down-regulation of MDR1 , thus indicating a central role of JNK signalling to suppress P-gp level in 5-Aza-treated Caki-1 cells .
	manualset3
110968	4	403150	5	NULL	NULL	0	NULL	down-regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , increased transcription activity of c-Jun by the JNK activation contributed to the down-regulation of MDR1 , thus indicating a central role of JNK signalling to suppress P-gp level in 5-Aza-treated Caki-1 cells .
	manualset3
110969	5	403150	5	NULL	NULL	0	NULL	MDR1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , increased transcription activity of c-Jun by the JNK activation contributed to the down-regulation of MDR1 , thus indicating a central role of JNK signalling to suppress P-gp level in 5-Aza-treated Caki-1 cells .
	manualset3
110970	6	403150	5	NULL	NULL	0	NULL	central role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , increased transcription activity of c-Jun by the JNK activation contributed to the down-regulation of MDR1 , thus indicating a central role of JNK signalling to suppress P-gp level in 5-Aza-treated Caki-1 cells .
	manualset3
110971	7	403150	5	NULL	NULL	0	NULL	JNK signalling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , increased transcription activity of c-Jun by the JNK activation contributed to the down-regulation of MDR1 , thus indicating a central role of JNK signalling to suppress P-gp level in 5-Aza-treated Caki-1 cells .
	manualset3
110972	8	403150	5	NULL	NULL	0	NULL	P-gp level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , increased transcription activity of c-Jun by the JNK activation contributed to the down-regulation of MDR1 , thus indicating a central role of JNK signalling to suppress P-gp level in 5-Aza-treated Caki-1 cells .
	manualset3
110973	9	403150	5	NULL	NULL	0	NULL	5-Aza-treated Caki-1 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , increased transcription activity of c-Jun by the JNK activation contributed to the down-regulation of MDR1 , thus indicating a central role of JNK signalling to suppress P-gp level in 5-Aza-treated Caki-1 cells .
	manualset3
111086	1	403151	5	NULL	NULL	NULL	NULL	inhibition 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Moreover , inhibition of E2F1 strongly reduced the expression of etoposide-induced HIC1 .
	manualset3
111087	2	403151	5	NULL	NULL	0	NULL	E2F1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , inhibition of E2F1 strongly reduced the expression of etoposide-induced HIC1 .
	manualset3
111088	3	403151	5	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , inhibition of E2F1 strongly reduced the expression of etoposide-induced HIC1 .
	manualset3
111089	4	403151	5	NULL	NULL	0	NULL	etoposide-induced HIC1	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , inhibition of E2F1 strongly reduced the expression of etoposide-induced HIC1 .
	manualset3
111090	1	403152	5	NULL	NULL	0	NULL	intracellular MnSOD	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , intracellular MnSOD was up-regulated by cytokines in osteoarthritis chondrocytes .
	manualset3
111091	2	403152	5	NULL	NULL	0	NULL	cytokines 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , intracellular MnSOD was up-regulated by cytokines in osteoarthritis chondrocytes .
	manualset3
111092	3	403152	5	NULL	NULL	0	NULL	osteoarthritis chondrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , intracellular MnSOD was up-regulated by cytokines in osteoarthritis chondrocytes .
	manualset3
111093	1	403153	5	NULL	NULL	0	NULL	sponge-adherent staphylococci	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , it appeared that in order to efficiently eradicate the sponge-adherent staphylococci the concentration of bacitracin 50-fold higher than the MBC value must be used .
	manualset3
111094	2	403153	5	NULL	NULL	0	NULL	concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , it appeared that in order to efficiently eradicate the sponge-adherent staphylococci the concentration of bacitracin 50-fold higher than the MBC value must be used .
	manualset3
111095	3	403153	5	NULL	NULL	0	NULL	bacitracin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , it appeared that in order to efficiently eradicate the sponge-adherent staphylococci the concentration of bacitracin 50-fold higher than the MBC value must be used .
	manualset3
111096	4	403153	5	NULL	NULL	0	NULL	MBC value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , it appeared that in order to efficiently eradicate the sponge-adherent staphylococci the concentration of bacitracin 50-fold higher than the MBC value must be used .
	manualset3
111097	1	403154	5	NULL	NULL	0	NULL	underrepresentation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , it is likely that underrepresentation of TDEE is most problematic in rural societies of the developing world which tend to have high activity levels and great risk of malnutrition .
	manualset3
111098	2	403154	5	NULL	NULL	0	NULL	TDEE 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , it is likely that underrepresentation of TDEE is most problematic in rural societies of the developing world which tend to have high activity levels and great risk of malnutrition .
	manualset3
111099	3	403154	5	NULL	NULL	0	NULL	rural societies	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , it is likely that underrepresentation of TDEE is most problematic in rural societies of the developing world which tend to have high activity levels and great risk of malnutrition .
	manualset3
111100	4	403154	5	NULL	NULL	0	NULL	developing world	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , it is likely that underrepresentation of TDEE is most problematic in rural societies of the developing world which tend to have high activity levels and great risk of malnutrition .
	manualset3
111101	5	403154	5	NULL	NULL	0	NULL	high activity levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , it is likely that underrepresentation of TDEE is most problematic in rural societies of the developing world which tend to have high activity levels and great risk of malnutrition .
	manualset3
111102	6	403154	5	NULL	NULL	0	NULL	risk 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , it is likely that underrepresentation of TDEE is most problematic in rural societies of the developing world which tend to have high activity levels and great risk of malnutrition .
	manualset3
111103	7	403154	5	NULL	NULL	0	NULL	malnutrition 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , it is likely that underrepresentation of TDEE is most problematic in rural societies of the developing world which tend to have high activity levels and great risk of malnutrition .
	manualset3
111104	1	403155	5	NULL	NULL	0	NULL	interaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , it was shown that the interaction of the AR with other proteins of the intracellular signal transduction cascade may promote prostate tumor growth .
	manualset3
111105	2	403155	5	NULL	NULL	0	NULL	AR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , it was shown that the interaction of the AR with other proteins of the intracellular signal transduction cascade may promote prostate tumor growth .
	manualset3
111106	3	403155	5	NULL	NULL	0	NULL	proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , it was shown that the interaction of the AR with other proteins of the intracellular signal transduction cascade may promote prostate tumor growth .
	manualset3
111107	4	403155	5	NULL	NULL	0	NULL	intracellular signal transduction cascade	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , it was shown that the interaction of the AR with other proteins of the intracellular signal transduction cascade may promote prostate tumor growth .
	manualset3
111108	5	403155	5	NULL	NULL	0	NULL	prostate tumor growth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , it was shown that the interaction of the AR with other proteins of the intracellular signal transduction cascade may promote prostate tumor growth .
	manualset3
111109	1	403156	5	NULL	NULL	0	NULL	levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , levels of the antioxidants superoxide dismutase ( SOD ) and glutathione ( GSH ) in Hep G2/SMP30 cells were a significant 42.6 % and 62.4 % lower than those in Hep G2/pcDNA3 cells , respectively .
	manualset3
111110	2	403156	5	NULL	NULL	0	NULL	antioxidants 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , levels of the antioxidants superoxide dismutase ( SOD ) and glutathione ( GSH ) in Hep G2/SMP30 cells were a significant 42.6 % and 62.4 % lower than those in Hep G2/pcDNA3 cells , respectively .
	manualset3
111111	3	403156	5	NULL	NULL	0	NULL	superoxide dismutase ( SOD )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , levels of the antioxidants superoxide dismutase ( SOD ) and glutathione ( GSH ) in Hep G2/SMP30 cells were a significant 42.6 % and 62.4 % lower than those in Hep G2/pcDNA3 cells , respectively .
	manualset3
111112	4	403156	5	NULL	NULL	0	NULL	glutathione ( GSH )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , levels of the antioxidants superoxide dismutase ( SOD ) and glutathione ( GSH ) in Hep G2/SMP30 cells were a significant 42.6 % and 62.4 % lower than those in Hep G2/pcDNA3 cells , respectively .
	manualset3
111113	5	403156	5	NULL	NULL	0	NULL	Hep G2/SMP30 cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , levels of the antioxidants superoxide dismutase ( SOD ) and glutathione ( GSH ) in Hep G2/SMP30 cells were a significant 42.6 % and 62.4 % lower than those in Hep G2/pcDNA3 cells , respectively .
	manualset3
111114	6	403156	5	NULL	NULL	0	NULL	42.6 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , levels of the antioxidants superoxide dismutase ( SOD ) and glutathione ( GSH ) in Hep G2/SMP30 cells were a significant 42.6 % and 62.4 % lower than those in Hep G2/pcDNA3 cells , respectively .
	manualset3
111115	7	403156	5	NULL	NULL	0	NULL	 62.4 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , levels of the antioxidants superoxide dismutase ( SOD ) and glutathione ( GSH ) in Hep G2/SMP30 cells were a significant 42.6 % and 62.4 % lower than those in Hep G2/pcDNA3 cells , respectively .
	manualset3
111116	8	403156	5	NULL	NULL	0	NULL	Hep G2/pcDNA3 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , levels of the antioxidants superoxide dismutase ( SOD ) and glutathione ( GSH ) in Hep G2/SMP30 cells were a significant 42.6 % and 62.4 % lower than those in Hep G2/pcDNA3 cells , respectively .
	manualset3
111117	1	403157	5	NULL	NULL	0	NULL	case study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A case study of the Raba River shows that incision has resulted from the increase in stream power caused by channelization and the simultaneous reduction in sediment supply due to variations in basin management and a change in flood hydrographs .
	manualset3
111118	2	403157	5	NULL	NULL	NULL	NULL	Raba River	GeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A case study of the Raba River shows that incision has resulted from the increase in stream power caused by channelization and the simultaneous reduction in sediment supply due to variations in basin management and a change in flood hydrographs .
	manualset3
111119	3	403157	5	NULL	NULL	0	NULL	incision 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A case study of the Raba River shows that incision has resulted from the increase in stream power caused by channelization and the simultaneous reduction in sediment supply due to variations in basin management and a change in flood hydrographs .
	manualset3
111120	4	403157	5	NULL	NULL	0	NULL	stream power	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A case study of the Raba River shows that incision has resulted from the increase in stream power caused by channelization and the simultaneous reduction in sediment supply due to variations in basin management and a change in flood hydrographs .
	manualset3
111121	5	403157	5	NULL	NULL	0	NULL	channelization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A case study of the Raba River shows that incision has resulted from the increase in stream power caused by channelization and the simultaneous reduction in sediment supply due to variations in basin management and a change in flood hydrographs .
	manualset3
111122	6	403157	5	NULL	NULL	0	NULL	simultaneous reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A case study of the Raba River shows that incision has resulted from the increase in stream power caused by channelization and the simultaneous reduction in sediment supply due to variations in basin management and a change in flood hydrographs .
	manualset3
111123	7	403157	5	NULL	NULL	0	NULL	sediment supply	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A case study of the Raba River shows that incision has resulted from the increase in stream power caused by channelization and the simultaneous reduction in sediment supply due to variations in basin management and a change in flood hydrographs .
	manualset3
111124	8	403157	5	NULL	NULL	0	NULL	variations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A case study of the Raba River shows that incision has resulted from the increase in stream power caused by channelization and the simultaneous reduction in sediment supply due to variations in basin management and a change in flood hydrographs .
	manualset3
111125	9	403157	5	NULL	NULL	0	NULL	basin management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A case study of the Raba River shows that incision has resulted from the increase in stream power caused by channelization and the simultaneous reduction in sediment supply due to variations in basin management and a change in flood hydrographs .
	manualset3
111126	10	403157	5	NULL	NULL	0	NULL	change 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A case study of the Raba River shows that incision has resulted from the increase in stream power caused by channelization and the simultaneous reduction in sediment supply due to variations in basin management and a change in flood hydrographs .
	manualset3
111127	11	403157	5	NULL	NULL	0	NULL	flood hydrographs	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A case study of the Raba River shows that incision has resulted from the increase in stream power caused by channelization and the simultaneous reduction in sediment supply due to variations in basin management and a change in flood hydrographs .
	manualset3
111128	1	403158	5	NULL	NULL	0	NULL	lung collagen hydroxyproline	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , lung collagen hydroxyproline , uronic acid , and hexosamine and also serum sialic acid , - glutamyltransferase ( GGT ) , and vascular endothelial growth factor ( VEGF ) levels were found to be significantly ( P & lt ; .001 ) lower in treated animals compared with untreated controls .
	manualset3
111129	2	403158	5	NULL	NULL	0	NULL	uronic acid	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , lung collagen hydroxyproline , uronic acid , and hexosamine and also serum sialic acid , - glutamyltransferase ( GGT ) , and vascular endothelial growth factor ( VEGF ) levels were found to be significantly ( P & lt ; .001 ) lower in treated animals compared with untreated controls .
	manualset3
111130	3	403158	5	NULL	NULL	0	NULL	hexosamine 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , lung collagen hydroxyproline , uronic acid , and hexosamine and also serum sialic acid , - glutamyltransferase ( GGT ) , and vascular endothelial growth factor ( VEGF ) levels were found to be significantly ( P & lt ; .001 ) lower in treated animals compared with untreated controls .
	manualset3
111131	4	403158	5	NULL	NULL	0	NULL	serum sialic acid	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , lung collagen hydroxyproline , uronic acid , and hexosamine and also serum sialic acid , - glutamyltransferase ( GGT ) , and vascular endothelial growth factor ( VEGF ) levels were found to be significantly ( P & lt ; .001 ) lower in treated animals compared with untreated controls .
	manualset3
111132	5	403158	5	NULL	NULL	0	NULL	-glutamyltransferase ( GGT )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , lung collagen hydroxyproline , uronic acid , and hexosamine and also serum sialic acid , - glutamyltransferase ( GGT ) , and vascular endothelial growth factor ( VEGF ) levels were found to be significantly ( P & lt ; .001 ) lower in treated animals compared with untreated controls .
	manualset3
111133	6	403158	5	NULL	NULL	0	NULL	vascular endothelial growth factor ( VEGF ) levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , lung collagen hydroxyproline , uronic acid , and hexosamine and also serum sialic acid , - glutamyltransferase ( GGT ) , and vascular endothelial growth factor ( VEGF ) levels were found to be significantly ( P & lt ; .001 ) lower in treated animals compared with untreated controls .
	manualset3
111134	7	403158	5	NULL	NULL	0	NULL	P & lt ; .001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , lung collagen hydroxyproline , uronic acid , and hexosamine and also serum sialic acid , - glutamyltransferase ( GGT ) , and vascular endothelial growth factor ( VEGF ) levels were found to be significantly ( P & lt ; .001 ) lower in treated animals compared with untreated controls .
	manualset3
111135	8	403158	5	NULL	NULL	0	NULL	treated animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , lung collagen hydroxyproline , uronic acid , and hexosamine and also serum sialic acid , - glutamyltransferase ( GGT ) , and vascular endothelial growth factor ( VEGF ) levels were found to be significantly ( P & lt ; .001 ) lower in treated animals compared with untreated controls .
	manualset3
111136	9	403158	5	NULL	NULL	0	NULL	untreated controls	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , lung collagen hydroxyproline , uronic acid , and hexosamine and also serum sialic acid , - glutamyltransferase ( GGT ) , and vascular endothelial growth factor ( VEGF ) levels were found to be significantly ( P & lt ; .001 ) lower in treated animals compared with untreated controls .
	manualset3
111137	1	403159	5	NULL	NULL	0	NULL	mature compost	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , mature compost did not produce any phytotoxic effect , behaving as a slow-action organic fertiliser with N made available through a progressive mineralisation .
	manualset3
111138	2	403159	5	NULL	NULL	0	NULL	phytotoxic effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , mature compost did not produce any phytotoxic effect , behaving as a slow-action organic fertiliser with N made available through a progressive mineralisation .
	manualset3
111139	3	403159	5	NULL	NULL	0	NULL	slow-action organic fertiliser	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , mature compost did not produce any phytotoxic effect , behaving as a slow-action organic fertiliser with N made available through a progressive mineralisation .
	manualset3
111140	4	403159	5	NULL	NULL	0	NULL	N	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , mature compost did not produce any phytotoxic effect , behaving as a slow-action organic fertiliser with N made available through a progressive mineralisation .
	manualset3
111141	5	403159	5	NULL	NULL	0	NULL	progressive mineralisation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , mature compost did not produce any phytotoxic effect , behaving as a slow-action organic fertiliser with N made available through a progressive mineralisation .
	manualset3
111142	1	403160	5	NULL	NULL	0	NULL	cancer cell phenotypes 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , mimicking cancer cell phenotypes by disrupting normal G ( 1 ) checkpoints sensitizes cells to PCC by ATR inhibition plus low-dose DNA damage .
	manualset3
111143	2	403160	5	NULL	NULL	0	NULL	normal G ( 1 ) checkpoints	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , mimicking cancer cell phenotypes by disrupting normal G ( 1 ) checkpoints sensitizes cells to PCC by ATR inhibition plus low-dose DNA damage .
	manualset3
111144	3	403160	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , mimicking cancer cell phenotypes by disrupting normal G ( 1 ) checkpoints sensitizes cells to PCC by ATR inhibition plus low-dose DNA damage .
	manualset3
111145	4	403160	5	NULL	NULL	0	NULL	PCC 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , mimicking cancer cell phenotypes by disrupting normal G ( 1 ) checkpoints sensitizes cells to PCC by ATR inhibition plus low-dose DNA damage .
	manualset3
111146	5	403160	5	NULL	NULL	0	NULL	ATR inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , mimicking cancer cell phenotypes by disrupting normal G ( 1 ) checkpoints sensitizes cells to PCC by ATR inhibition plus low-dose DNA damage .
	manualset3
111147	6	403160	5	NULL	NULL	0	NULL	low-dose DNA damage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , mimicking cancer cell phenotypes by disrupting normal G ( 1 ) checkpoints sensitizes cells to PCC by ATR inhibition plus low-dose DNA damage .
	manualset3
111148	1	403161	5	NULL	NULL	0	NULL	neurons 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , neurons in lateral intraparietal cortex ( LIP ) continue to remap information across hemifields in the absence of the forebrain commissures .
	manualset3
111149	2	403161	5	NULL	NULL	0	NULL	lateral intraparietal cortex ( LIP )	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , neurons in lateral intraparietal cortex ( LIP ) continue to remap information across hemifields in the absence of the forebrain commissures .
	manualset3
111150	3	403161	5	NULL	NULL	0	NULL	information 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , neurons in lateral intraparietal cortex ( LIP ) continue to remap information across hemifields in the absence of the forebrain commissures .
	manualset3
111151	4	403161	5	NULL	NULL	0	NULL	hemifields 	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , neurons in lateral intraparietal cortex ( LIP ) continue to remap information across hemifields in the absence of the forebrain commissures .
	manualset3
111152	5	403161	5	NULL	NULL	0	NULL	absence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , neurons in lateral intraparietal cortex ( LIP ) continue to remap information across hemifields in the absence of the forebrain commissures .
	manualset3
111153	6	403161	5	NULL	NULL	0	NULL	forebrain commissures	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , neurons in lateral intraparietal cortex ( LIP ) continue to remap information across hemifields in the absence of the forebrain commissures .
	manualset3
111154	1	403162	5	NULL	NULL	0	NULL	obesity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , obesity can play a role in the prognosis of certain cancers .
	manualset3
111155	2	403162	5	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , obesity can play a role in the prognosis of certain cancers .
	manualset3
111156	3	403162	5	NULL	NULL	0	NULL	prognosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , obesity can play a role in the prognosis of certain cancers .
	manualset3
111157	4	403162	5	NULL	NULL	0	NULL	cancers 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , obesity can play a role in the prognosis of certain cancers .
	manualset3
111158	1	403163	5	NULL	NULL	0	NULL	trial-recall curves	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , on the trial-recall curves , from the first trial to the last two groups showed no significant differences in their learning effect and forgetting .
	manualset3
111159	2	403163	5	NULL	NULL	0	NULL	first trial	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , on the trial-recall curves , from the first trial to the last two groups showed no significant differences in their learning effect and forgetting .
	manualset3
111160	3	403163	5	NULL	NULL	0	NULL	two groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , on the trial-recall curves , from the first trial to the last two groups showed no significant differences in their learning effect and forgetting .
	manualset3
111161	4	403163	5	NULL	NULL	0	NULL	significant differences 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , on the trial-recall curves , from the first trial to the last two groups showed no significant differences in their learning effect and forgetting .
	manualset3
111162	5	403163	5	NULL	NULL	0	NULL	learning effect	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , on the trial-recall curves , from the first trial to the last two groups showed no significant differences in their learning effect and forgetting .
	manualset3
111163	6	403163	5	NULL	NULL	0	NULL	forgetting 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , on the trial-recall curves , from the first trial to the last two groups showed no significant differences in their learning effect and forgetting .
	manualset3
111164	1	403164	5	NULL	NULL	0	NULL	oncogenic mutations 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , oncogenic mutations in RAS or B-RAF are responsible for a large proportion of human cancers .
	manualset3
111165	2	403164	5	NULL	NULL	0	NULL	RAS 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , oncogenic mutations in RAS or B-RAF are responsible for a large proportion of human cancers .
	manualset3
111166	3	403164	5	NULL	NULL	0	NULL	B-RAF	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , oncogenic mutations in RAS or B-RAF are responsible for a large proportion of human cancers .
	manualset3
111167	4	403164	5	NULL	NULL	0	NULL	large proportion 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , oncogenic mutations in RAS or B-RAF are responsible for a large proportion of human cancers .
	manualset3
111168	5	403164	5	NULL	NULL	0	NULL	human cancers	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , oncogenic mutations in RAS or B-RAF are responsible for a large proportion of human cancers .
	manualset3
111169	1	403165	5	NULL	NULL	0	NULL	organically cultured seeds	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , organically and conventionally cultured seeds were employed to determine whether the seed provenance influenced the test sensitivity .
	manualset3
111170	2	403165	5	NULL	NULL	0	NULL	conventionally cultured seeds	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , organically and conventionally cultured seeds were employed to determine whether the seed provenance influenced the test sensitivity .
	manualset3
111171	3	403165	5	NULL	NULL	0	NULL	seed provenance	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , organically and conventionally cultured seeds were employed to determine whether the seed provenance influenced the test sensitivity .
	manualset3
111172	4	403165	5	NULL	NULL	0	NULL	test sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , organically and conventionally cultured seeds were employed to determine whether the seed provenance influenced the test sensitivity .
	manualset3
111173	1	403166	5	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , our previous study demonstrated a beneficial effect of an extracorporeal device to increase the oxygenated blood to the liver and to improve the survival rate of animals subjected to subtotal hepatectomy .
	manualset3
111174	2	403166	5	NULL	NULL	0	NULL	beneficial effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , our previous study demonstrated a beneficial effect of an extracorporeal device to increase the oxygenated blood to the liver and to improve the survival rate of animals subjected to subtotal hepatectomy .
	manualset3
111175	3	403166	5	NULL	NULL	0	NULL	extracorporeal device	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , our previous study demonstrated a beneficial effect of an extracorporeal device to increase the oxygenated blood to the liver and to improve the survival rate of animals subjected to subtotal hepatectomy .
	manualset3
111176	4	403166	5	NULL	NULL	0	NULL	oxygenated blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , our previous study demonstrated a beneficial effect of an extracorporeal device to increase the oxygenated blood to the liver and to improve the survival rate of animals subjected to subtotal hepatectomy .
	manualset3
111177	5	403166	5	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , our previous study demonstrated a beneficial effect of an extracorporeal device to increase the oxygenated blood to the liver and to improve the survival rate of animals subjected to subtotal hepatectomy .
	manualset3
111178	6	403166	5	NULL	NULL	0	NULL	survival rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , our previous study demonstrated a beneficial effect of an extracorporeal device to increase the oxygenated blood to the liver and to improve the survival rate of animals subjected to subtotal hepatectomy .
	manualset3
111179	7	403166	5	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , our previous study demonstrated a beneficial effect of an extracorporeal device to increase the oxygenated blood to the liver and to improve the survival rate of animals subjected to subtotal hepatectomy .
	manualset3
111180	8	403166	5	NULL	NULL	0	NULL	subtotal hepatectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , our previous study demonstrated a beneficial effect of an extracorporeal device to increase the oxygenated blood to the liver and to improve the survival rate of animals subjected to subtotal hepatectomy .
	manualset3
111181	1	403167	5	NULL	NULL	0	NULL	cataract	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A cataract is a clouding of the crystalline lens that reduces the amount of incoming light and impairs visual perception .
	manualset3
111182	2	403167	5	NULL	NULL	0	NULL	crystalline lens	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A cataract is a clouding of the crystalline lens that reduces the amount of incoming light and impairs visual perception .
	manualset3
111183	3	403167	5	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A cataract is a clouding of the crystalline lens that reduces the amount of incoming light and impairs visual perception .
	manualset3
111184	4	403167	5	NULL	NULL	0	NULL	incoming light	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A cataract is a clouding of the crystalline lens that reduces the amount of incoming light and impairs visual perception .
	manualset3
111185	5	403167	5	NULL	NULL	0	NULL	visual perception	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A cataract is a clouding of the crystalline lens that reduces the amount of incoming light and impairs visual perception .
	manualset3
122142	6	403167	5	NULL	NULL	0	NULL	clouding 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A cataract is a clouding of the crystalline lens that reduces the amount of incoming light and impairs visual perception .
	manualset3
111186	1	403168	5	NULL	NULL	0	NULL	performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , performance on discrimination but not detection , correlated with performance on mathematics .
	manualset3
111187	2	403168	5	NULL	NULL	0	NULL	discrimination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , performance on discrimination but not detection , correlated with performance on mathematics .
	manualset3
111188	3	403168	5	NULL	NULL	0	NULL	detection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , performance on discrimination but not detection , correlated with performance on mathematics .
	manualset3
111189	4	403168	5	NULL	NULL	0	NULL	performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , performance on discrimination but not detection , correlated with performance on mathematics .
	manualset3
111190	5	403168	5	NULL	NULL	0	NULL	mathematics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , performance on discrimination but not detection , correlated with performance on mathematics .
	manualset3
111191	1	403169	5	NULL	NULL	0	NULL	rapamycin treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , rapamycin treatment also enhanced the level of stem cell-associated genes and CD133 expression in certain human liver tumor cell lines , such as Huh7 , PLC/PRC/7 and Hep3B .
	manualset3
111192	2	403169	5	NULL	NULL	0	NULL	level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , rapamycin treatment also enhanced the level of stem cell-associated genes and CD133 expression in certain human liver tumor cell lines , such as Huh7 , PLC/PRC/7 and Hep3B .
	manualset3
111193	3	403169	5	NULL	NULL	0	NULL	stem cell-associated genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , rapamycin treatment also enhanced the level of stem cell-associated genes and CD133 expression in certain human liver tumor cell lines , such as Huh7 , PLC/PRC/7 and Hep3B .
	manualset3
111194	4	403169	5	NULL	NULL	0	NULL	CD133 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , rapamycin treatment also enhanced the level of stem cell-associated genes and CD133 expression in certain human liver tumor cell lines , such as Huh7 , PLC/PRC/7 and Hep3B .
	manualset3
111195	5	403169	5	NULL	NULL	0	NULL	human liver tumor cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , rapamycin treatment also enhanced the level of stem cell-associated genes and CD133 expression in certain human liver tumor cell lines , such as Huh7 , PLC/PRC/7 and Hep3B .
	manualset3
111196	6	403169	5	NULL	NULL	0	NULL	Huh7	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , rapamycin treatment also enhanced the level of stem cell-associated genes and CD133 expression in certain human liver tumor cell lines , such as Huh7 , PLC/PRC/7 and Hep3B .
	manualset3
111197	7	403169	5	NULL	NULL	0	NULL	PLC/PRC/7	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , rapamycin treatment also enhanced the level of stem cell-associated genes and CD133 expression in certain human liver tumor cell lines , such as Huh7 , PLC/PRC/7 and Hep3B .
	manualset3
111198	8	403169	5	NULL	NULL	0	NULL	Hep3B	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , rapamycin treatment also enhanced the level of stem cell-associated genes and CD133 expression in certain human liver tumor cell lines , such as Huh7 , PLC/PRC/7 and Hep3B .
	manualset3
111199	1	403170	5	NULL	NULL	0	NULL	resveratrol treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , resveratrol treatment modulated the differentiation of morphological characteristics including elongation and cell fusion in cardiomyoblasts .
	manualset3
111200	2	403170	5	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , resveratrol treatment modulated the differentiation of morphological characteristics including elongation and cell fusion in cardiomyoblasts .
	manualset3
111201	3	403170	5	NULL	NULL	0	NULL	morphological characteristics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , resveratrol treatment modulated the differentiation of morphological characteristics including elongation and cell fusion in cardiomyoblasts .
	manualset3
111202	4	403170	5	NULL	NULL	0	NULL	elongation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , resveratrol treatment modulated the differentiation of morphological characteristics including elongation and cell fusion in cardiomyoblasts .
	manualset3
111203	5	403170	5	NULL	NULL	0	NULL	cell fusion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , resveratrol treatment modulated the differentiation of morphological characteristics including elongation and cell fusion in cardiomyoblasts .
	manualset3
111204	6	403170	5	NULL	NULL	0	NULL	cardiomyoblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , resveratrol treatment modulated the differentiation of morphological characteristics including elongation and cell fusion in cardiomyoblasts .
	manualset3
111205	1	403171	5	NULL	NULL	0	NULL	cell-surface interactions 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , specific cell-surface interactions are promoted due to reduced shear , allowing gentle cell rolling and arrest .
	manualset3
111206	2	403171	5	NULL	NULL	0	NULL	reduced shear	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , specific cell-surface interactions are promoted due to reduced shear , allowing gentle cell rolling and arrest .
	manualset3
122143	3	403171	5	NULL	NULL	0	NULL	cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , specific cell-surface interactions are promoted due to reduced shear , allowing gentle cell rolling and arrest .
	manualset3
111207	1	403172	5	NULL	NULL	0	NULL	stress fibers	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , stress fibers were identified in human thyroid papillary carcinoma cell lines harboring RET/PTC1 rearrangements but not in thyroid carcinoma cells negative for RET/PTC rearrangements .
	manualset3
111208	2	403172	5	NULL	NULL	0	NULL	human thyroid papillary carcinoma cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , stress fibers were identified in human thyroid papillary carcinoma cell lines harboring RET/PTC1 rearrangements but not in thyroid carcinoma cells negative for RET/PTC rearrangements .
	manualset3
111209	3	403172	5	NULL	NULL	0	NULL	RET/PTC1 rearrangements	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , stress fibers were identified in human thyroid papillary carcinoma cell lines harboring RET/PTC1 rearrangements but not in thyroid carcinoma cells negative for RET/PTC rearrangements .
	manualset3
111210	4	403172	5	NULL	NULL	0	NULL	thyroid carcinoma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , stress fibers were identified in human thyroid papillary carcinoma cell lines harboring RET/PTC1 rearrangements but not in thyroid carcinoma cells negative for RET/PTC rearrangements .
	manualset3
111211	5	403172	5	NULL	NULL	0	NULL	RET/PTC rearrangements	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , stress fibers were identified in human thyroid papillary carcinoma cell lines harboring RET/PTC1 rearrangements but not in thyroid carcinoma cells negative for RET/PTC rearrangements .
	manualset3
111212	1	403173	5	NULL	NULL	0	NULL	C terminus	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the C terminus of tau clearly inhibits the assembly process ; this inhibition can be partially reversed by site-specific phosphorylation and completely removed by truncation events at various sites from S ( 320 ) to the end of the molecule .
	manualset3
111213	2	403173	5	NULL	NULL	0	NULL	tau	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the C terminus of tau clearly inhibits the assembly process ; this inhibition can be partially reversed by site-specific phosphorylation and completely removed by truncation events at various sites from S ( 320 ) to the end of the molecule .
	manualset3
111214	3	403173	5	NULL	NULL	0	NULL	assembly process	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the C terminus of tau clearly inhibits the assembly process ; this inhibition can be partially reversed by site-specific phosphorylation and completely removed by truncation events at various sites from S ( 320 ) to the end of the molecule .
	manualset3
111215	4	403173	5	NULL	NULL	0	NULL	inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the C terminus of tau clearly inhibits the assembly process ; this inhibition can be partially reversed by site-specific phosphorylation and completely removed by truncation events at various sites from S ( 320 ) to the end of the molecule .
	manualset3
111217	5	403173	5	NULL	NULL	0	NULL	site-specific phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the C terminus of tau clearly inhibits the assembly process ; this inhibition can be partially reversed by site-specific phosphorylation and completely removed by truncation events at various sites from S ( 320 ) to the end of the molecule .
	manualset3
111218	6	403173	5	NULL	NULL	0	NULL	truncation events	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the C terminus of tau clearly inhibits the assembly process ; this inhibition can be partially reversed by site-specific phosphorylation and completely removed by truncation events at various sites from S ( 320 ) to the end of the molecule .
	manualset3
111220	7	403173	5	NULL	NULL	0	NULL	various sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the C terminus of tau clearly inhibits the assembly process ; this inhibition can be partially reversed by site-specific phosphorylation and completely removed by truncation events at various sites from S ( 320 ) to the end of the molecule .
	manualset3
111221	8	403173	5	NULL	NULL	0	NULL	S ( 320 )	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the C terminus of tau clearly inhibits the assembly process ; this inhibition can be partially reversed by site-specific phosphorylation and completely removed by truncation events at various sites from S ( 320 ) to the end of the molecule .
	manualset3
111222	9	403173	5	NULL	NULL	0	NULL	molecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the C terminus of tau clearly inhibits the assembly process ; this inhibition can be partially reversed by site-specific phosphorylation and completely removed by truncation events at various sites from S ( 320 ) to the end of the molecule .
	manualset3
111231	1	403174	5	NULL	NULL	0	NULL	CL intensities	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the CL intensities improved regularly with increasing carbon chain length of the dicarboxylic acids .
	manualset3
111232	2	403174	5	NULL	NULL	0	NULL	carbon chain length	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the CL intensities improved regularly with increasing carbon chain length of the dicarboxylic acids .
	manualset3
111234	3	403174	5	NULL	NULL	0	NULL	dicarboxylic acids	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the CL intensities improved regularly with increasing carbon chain length of the dicarboxylic acids .
	manualset3
111237	1	403175	5	NULL	NULL	0	NULL	MR	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the MR tends to follow a logH behavior at high fields .
	manualset3
111241	2	403175	5	NULL	NULL	0	NULL	logH behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the MR tends to follow a logH behavior at high fields .
	manualset3
111242	3	403175	5	NULL	NULL	0	NULL	high fields	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the MR tends to follow a logH behavior at high fields .
	manualset3
111248	1	403176	5	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the absence of inhibition of ornithynedecarboxylase activity by high levels of putrescine is noted .
	manualset3
111250	2	403176	5	NULL	NULL	0	NULL	inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the absence of inhibition of ornithynedecarboxylase activity by high levels of putrescine is noted .
	manualset3
111253	3	403176	5	NULL	NULL	0	NULL	ornithynedecarboxylase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the absence of inhibition of ornithynedecarboxylase activity by high levels of putrescine is noted .
	manualset3
111255	4	403176	5	NULL	NULL	0	NULL	high levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the absence of inhibition of ornithynedecarboxylase activity by high levels of putrescine is noted .
	manualset3
111256	5	403176	5	NULL	NULL	0	NULL	putrescine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the absence of inhibition of ornithynedecarboxylase activity by high levels of putrescine is noted .
	manualset3
111258	1	403177	5	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the addition of NG-monomethyl-L-arginine ( NMMA ) to Con A-stimulated splenocyte cultures attenuates the suppressive effect of morphine on mitogenic responsiveness .
	manualset3
111260	2	403177	5	NULL	NULL	0	NULL	NG-monomethyl-L-arginine ( NMMA )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the addition of NG-monomethyl-L-arginine ( NMMA ) to Con A-stimulated splenocyte cultures attenuates the suppressive effect of morphine on mitogenic responsiveness .
	manualset3
111263	3	403177	5	NULL	NULL	0	NULL	Con A-stimulated splenocyte cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the addition of NG-monomethyl-L-arginine ( NMMA ) to Con A-stimulated splenocyte cultures attenuates the suppressive effect of morphine on mitogenic responsiveness .
	manualset3
111266	4	403177	5	NULL	NULL	0	NULL	suppressive effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the addition of NG-monomethyl-L-arginine ( NMMA ) to Con A-stimulated splenocyte cultures attenuates the suppressive effect of morphine on mitogenic responsiveness .
	manualset3
111268	5	403177	5	NULL	NULL	0	NULL	morphine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the addition of NG-monomethyl-L-arginine ( NMMA ) to Con A-stimulated splenocyte cultures attenuates the suppressive effect of morphine on mitogenic responsiveness .
	manualset3
111269	6	403177	5	NULL	NULL	0	NULL	mitogenic responsiveness	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the addition of NG-monomethyl-L-arginine ( NMMA ) to Con A-stimulated splenocyte cultures attenuates the suppressive effect of morphine on mitogenic responsiveness .
	manualset3
111270	1	403178	5	NULL	NULL	0	NULL	atrioventricular node	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the atrioventricular node protects the ventricles from rapid atrial arrhythmias and may take over pacemaker function when the sinus node fails .
	manualset3
111271	2	403178	5	NULL	NULL	0	NULL	ventricles	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the atrioventricular node protects the ventricles from rapid atrial arrhythmias and may take over pacemaker function when the sinus node fails .
	manualset3
111272	3	403178	5	NULL	NULL	0	NULL	rapid atrial arrhythmias	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the atrioventricular node protects the ventricles from rapid atrial arrhythmias and may take over pacemaker function when the sinus node fails .
	manualset3
111274	4	403178	5	NULL	NULL	NULL	NULL	pacemaker function	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Moreover , the atrioventricular node protects the ventricles from rapid atrial arrhythmias and may take over pacemaker function when the sinus node fails .
	manualset3
111276	5	403178	5	NULL	NULL	0	NULL	sinus node	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the atrioventricular node protects the ventricles from rapid atrial arrhythmias and may take over pacemaker function when the sinus node fails .
	manualset3
111290	1	403179	5	NULL	NULL	0	NULL	semen quality	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the effect on semen quality following centrifugation was assessed by monitoring several sperm parameters ( membrane integrity using SYBR14-PI , acrosomal status using PSA-FITC , percentage total motility ( TM ) , percentage progressive motility ( PM ) and beat cross frequency ( BCF ) obtained with computer assisted sperm analysis ( CASA ) ) immediately after centrifugation and daily during chilled storage for 3 d. The use of CP1 resulted in a sperm loss of 22 % .
	manualset3
111386	2	403179	5	NULL	NULL	0	NULL	centrifugation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the effect on semen quality following centrifugation was assessed by monitoring several sperm parameters ( membrane integrity using SYBR14-PI , acrosomal status using PSA-FITC , percentage total motility ( TM ) , percentage progressive motility ( PM ) and beat cross frequency ( BCF ) obtained with computer assisted sperm analysis ( CASA ) ) immediately after centrifugation and daily during chilled storage for 3 d. The use of CP1 resulted in a sperm loss of 22 % .
	manualset3
111387	3	403179	5	NULL	NULL	0	NULL	sperm parameters	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the effect on semen quality following centrifugation was assessed by monitoring several sperm parameters ( membrane integrity using SYBR14-PI , acrosomal status using PSA-FITC , percentage total motility ( TM ) , percentage progressive motility ( PM ) and beat cross frequency ( BCF ) obtained with computer assisted sperm analysis ( CASA ) ) immediately after centrifugation and daily during chilled storage for 3 d. The use of CP1 resulted in a sperm loss of 22 % .
	manualset3
111388	4	403179	5	NULL	NULL	0	NULL	membrane integrity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the effect on semen quality following centrifugation was assessed by monitoring several sperm parameters ( membrane integrity using SYBR14-PI , acrosomal status using PSA-FITC , percentage total motility ( TM ) , percentage progressive motility ( PM ) and beat cross frequency ( BCF ) obtained with computer assisted sperm analysis ( CASA ) ) immediately after centrifugation and daily during chilled storage for 3 d. The use of CP1 resulted in a sperm loss of 22 % .
	manualset3
111389	5	403179	5	NULL	NULL	0	NULL	SYBR14-PI	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the effect on semen quality following centrifugation was assessed by monitoring several sperm parameters ( membrane integrity using SYBR14-PI , acrosomal status using PSA-FITC , percentage total motility ( TM ) , percentage progressive motility ( PM ) and beat cross frequency ( BCF ) obtained with computer assisted sperm analysis ( CASA ) ) immediately after centrifugation and daily during chilled storage for 3 d. The use of CP1 resulted in a sperm loss of 22 % .
	manualset3
111390	6	403179	5	NULL	NULL	0	NULL	acrosomal status	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the effect on semen quality following centrifugation was assessed by monitoring several sperm parameters ( membrane integrity using SYBR14-PI , acrosomal status using PSA-FITC , percentage total motility ( TM ) , percentage progressive motility ( PM ) and beat cross frequency ( BCF ) obtained with computer assisted sperm analysis ( CASA ) ) immediately after centrifugation and daily during chilled storage for 3 d. The use of CP1 resulted in a sperm loss of 22 % .
	manualset3
111391	7	403179	5	NULL	NULL	0	NULL	PSA-FITC	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the effect on semen quality following centrifugation was assessed by monitoring several sperm parameters ( membrane integrity using SYBR14-PI , acrosomal status using PSA-FITC , percentage total motility ( TM ) , percentage progressive motility ( PM ) and beat cross frequency ( BCF ) obtained with computer assisted sperm analysis ( CASA ) ) immediately after centrifugation and daily during chilled storage for 3 d. The use of CP1 resulted in a sperm loss of 22 % .
	manualset3
111392	8	403179	5	NULL	NULL	0	NULL	percentage total motility ( TM )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the effect on semen quality following centrifugation was assessed by monitoring several sperm parameters ( membrane integrity using SYBR14-PI , acrosomal status using PSA-FITC , percentage total motility ( TM ) , percentage progressive motility ( PM ) and beat cross frequency ( BCF ) obtained with computer assisted sperm analysis ( CASA ) ) immediately after centrifugation and daily during chilled storage for 3 d. The use of CP1 resulted in a sperm loss of 22 % .
	manualset3
111393	9	403179	5	NULL	NULL	0	NULL	percentage progressive motility ( PM )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the effect on semen quality following centrifugation was assessed by monitoring several sperm parameters ( membrane integrity using SYBR14-PI , acrosomal status using PSA-FITC , percentage total motility ( TM ) , percentage progressive motility ( PM ) and beat cross frequency ( BCF ) obtained with computer assisted sperm analysis ( CASA ) ) immediately after centrifugation and daily during chilled storage for 3 d. The use of CP1 resulted in a sperm loss of 22 % .
	manualset3
111394	10	403179	5	NULL	NULL	0	NULL	beat cross frequency ( BCF )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the effect on semen quality following centrifugation was assessed by monitoring several sperm parameters ( membrane integrity using SYBR14-PI , acrosomal status using PSA-FITC , percentage total motility ( TM ) , percentage progressive motility ( PM ) and beat cross frequency ( BCF ) obtained with computer assisted sperm analysis ( CASA ) ) immediately after centrifugation and daily during chilled storage for 3 d. The use of CP1 resulted in a sperm loss of 22 % .
	manualset3
111395	11	403179	5	NULL	NULL	0	NULL	computer assisted sperm analysis ( CASA )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the effect on semen quality following centrifugation was assessed by monitoring several sperm parameters ( membrane integrity using SYBR14-PI , acrosomal status using PSA-FITC , percentage total motility ( TM ) , percentage progressive motility ( PM ) and beat cross frequency ( BCF ) obtained with computer assisted sperm analysis ( CASA ) ) immediately after centrifugation and daily during chilled storage for 3 d. The use of CP1 resulted in a sperm loss of 22 % .
	manualset3
111396	12	403179	5	NULL	NULL	0	NULL	centrifugation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the effect on semen quality following centrifugation was assessed by monitoring several sperm parameters ( membrane integrity using SYBR14-PI , acrosomal status using PSA-FITC , percentage total motility ( TM ) , percentage progressive motility ( PM ) and beat cross frequency ( BCF ) obtained with computer assisted sperm analysis ( CASA ) ) immediately after centrifugation and daily during chilled storage for 3 d. The use of CP1 resulted in a sperm loss of 22 % .
	manualset3
111397	13	403179	5	NULL	NULL	0	NULL	chilled storage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the effect on semen quality following centrifugation was assessed by monitoring several sperm parameters ( membrane integrity using SYBR14-PI , acrosomal status using PSA-FITC , percentage total motility ( TM ) , percentage progressive motility ( PM ) and beat cross frequency ( BCF ) obtained with computer assisted sperm analysis ( CASA ) ) immediately after centrifugation and daily during chilled storage for 3 d. The use of CP1 resulted in a sperm loss of 22 % .
	manualset3
111398	14	403179	5	NULL	NULL	0	NULL	3 d	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the effect on semen quality following centrifugation was assessed by monitoring several sperm parameters ( membrane integrity using SYBR14-PI , acrosomal status using PSA-FITC , percentage total motility ( TM ) , percentage progressive motility ( PM ) and beat cross frequency ( BCF ) obtained with computer assisted sperm analysis ( CASA ) ) immediately after centrifugation and daily during chilled storage for 3 d. The use of CP1 resulted in a sperm loss of 22 % .
	manualset3
111399	15	403179	5	NULL	NULL	0	NULL	CP1	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the effect on semen quality following centrifugation was assessed by monitoring several sperm parameters ( membrane integrity using SYBR14-PI , acrosomal status using PSA-FITC , percentage total motility ( TM ) , percentage progressive motility ( PM ) and beat cross frequency ( BCF ) obtained with computer assisted sperm analysis ( CASA ) ) immediately after centrifugation and daily during chilled storage for 3 d. The use of CP1 resulted in a sperm loss of 22 % .
	manualset3
111400	16	403179	5	NULL	NULL	0	NULL	sperm loss	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the effect on semen quality following centrifugation was assessed by monitoring several sperm parameters ( membrane integrity using SYBR14-PI , acrosomal status using PSA-FITC , percentage total motility ( TM ) , percentage progressive motility ( PM ) and beat cross frequency ( BCF ) obtained with computer assisted sperm analysis ( CASA ) ) immediately after centrifugation and daily during chilled storage for 3 d. The use of CP1 resulted in a sperm loss of 22 % .
	manualset3
111401	17	403179	5	NULL	NULL	0	NULL	22 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the effect on semen quality following centrifugation was assessed by monitoring several sperm parameters ( membrane integrity using SYBR14-PI , acrosomal status using PSA-FITC , percentage total motility ( TM ) , percentage progressive motility ( PM ) and beat cross frequency ( BCF ) obtained with computer assisted sperm analysis ( CASA ) ) immediately after centrifugation and daily during chilled storage for 3 d. The use of CP1 resulted in a sperm loss of 22 % .
	manualset3
111402	1	403180	5	NULL	NULL	0	NULL	CK response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the enhancing CK response in rat tissues was specific to anti-E2 15 plus E2 since the intact anti-E2 in the presence of other estrogen mimetics , such as oestriol or stilbestrol or tamoxifen did not potentiate the CK response in rat tissues .
	manualset3
111403	2	403180	5	NULL	NULL	0	NULL	rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the enhancing CK response in rat tissues was specific to anti-E2 15 plus E2 since the intact anti-E2 in the presence of other estrogen mimetics , such as oestriol or stilbestrol or tamoxifen did not potentiate the CK response in rat tissues .
	manualset3
111404	3	403180	5	NULL	NULL	0	NULL	tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the enhancing CK response in rat tissues was specific to anti-E2 15 plus E2 since the intact anti-E2 in the presence of other estrogen mimetics , such as oestriol or stilbestrol or tamoxifen did not potentiate the CK response in rat tissues .
	manualset3
111405	4	403180	5	NULL	NULL	0	NULL	anti-E2 15 plus E2	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the enhancing CK response in rat tissues was specific to anti-E2 15 plus E2 since the intact anti-E2 in the presence of other estrogen mimetics , such as oestriol or stilbestrol or tamoxifen did not potentiate the CK response in rat tissues .
	manualset3
111406	5	403180	5	NULL	NULL	0	NULL	anti-E2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the enhancing CK response in rat tissues was specific to anti-E2 15 plus E2 since the intact anti-E2 in the presence of other estrogen mimetics , such as oestriol or stilbestrol or tamoxifen did not potentiate the CK response in rat tissues .
	manualset3
111407	6	403180	5	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the enhancing CK response in rat tissues was specific to anti-E2 15 plus E2 since the intact anti-E2 in the presence of other estrogen mimetics , such as oestriol or stilbestrol or tamoxifen did not potentiate the CK response in rat tissues .
	manualset3
111408	7	403180	5	NULL	NULL	0	NULL	estrogen mimetics	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the enhancing CK response in rat tissues was specific to anti-E2 15 plus E2 since the intact anti-E2 in the presence of other estrogen mimetics , such as oestriol or stilbestrol or tamoxifen did not potentiate the CK response in rat tissues .
	manualset3
111409	8	403180	5	NULL	NULL	0	NULL	oestriol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the enhancing CK response in rat tissues was specific to anti-E2 15 plus E2 since the intact anti-E2 in the presence of other estrogen mimetics , such as oestriol or stilbestrol or tamoxifen did not potentiate the CK response in rat tissues .
	manualset3
111410	9	403180	5	NULL	NULL	0	NULL	stilbestrol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the enhancing CK response in rat tissues was specific to anti-E2 15 plus E2 since the intact anti-E2 in the presence of other estrogen mimetics , such as oestriol or stilbestrol or tamoxifen did not potentiate the CK response in rat tissues .
	manualset3
111411	10	403180	5	NULL	NULL	0	NULL	tamoxifen	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the enhancing CK response in rat tissues was specific to anti-E2 15 plus E2 since the intact anti-E2 in the presence of other estrogen mimetics , such as oestriol or stilbestrol or tamoxifen did not potentiate the CK response in rat tissues .
	manualset3
111412	11	403180	5	NULL	NULL	0	NULL	CK response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the enhancing CK response in rat tissues was specific to anti-E2 15 plus E2 since the intact anti-E2 in the presence of other estrogen mimetics , such as oestriol or stilbestrol or tamoxifen did not potentiate the CK response in rat tissues .
	manualset3
111413	12	403180	5	NULL	NULL	0	NULL	rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the enhancing CK response in rat tissues was specific to anti-E2 15 plus E2 since the intact anti-E2 in the presence of other estrogen mimetics , such as oestriol or stilbestrol or tamoxifen did not potentiate the CK response in rat tissues .
	manualset3
111414	13	403180	5	NULL	NULL	0	NULL	tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the enhancing CK response in rat tissues was specific to anti-E2 15 plus E2 since the intact anti-E2 in the presence of other estrogen mimetics , such as oestriol or stilbestrol or tamoxifen did not potentiate the CK response in rat tissues .
	manualset3
111415	1	403181	5	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the expression of three endoderm-specific genes , GATA6 , HNF4 , and Dab2 , is down-regulated in TIF1beta ( HP1box / - ) cells compared with wild-type cells during PrE differentiation .
	manualset3
111416	2	403181	5	NULL	NULL	0	NULL	endoderm-specific genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the expression of three endoderm-specific genes , GATA6 , HNF4 , and Dab2 , is down-regulated in TIF1beta ( HP1box / - ) cells compared with wild-type cells during PrE differentiation .
	manualset3
111417	3	403181	5	NULL	NULL	0	NULL	GATA6	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the expression of three endoderm-specific genes , GATA6 , HNF4 , and Dab2 , is down-regulated in TIF1beta ( HP1box / - ) cells compared with wild-type cells during PrE differentiation .
	manualset3
111418	4	403181	5	NULL	NULL	0	NULL	HNF4	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the expression of three endoderm-specific genes , GATA6 , HNF4 , and Dab2 , is down-regulated in TIF1beta ( HP1box / - ) cells compared with wild-type cells during PrE differentiation .
	manualset3
111419	5	403181	5	NULL	NULL	0	NULL	Dab2	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the expression of three endoderm-specific genes , GATA6 , HNF4 , and Dab2 , is down-regulated in TIF1beta ( HP1box / - ) cells compared with wild-type cells during PrE differentiation .
	manualset3
111420	6	403181	5	NULL	NULL	0	NULL	TIF1beta ( HP1box / - ) cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the expression of three endoderm-specific genes , GATA6 , HNF4 , and Dab2 , is down-regulated in TIF1beta ( HP1box / - ) cells compared with wild-type cells during PrE differentiation .
	manualset3
111421	7	403181	5	NULL	NULL	0	NULL	wild-type cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the expression of three endoderm-specific genes , GATA6 , HNF4 , and Dab2 , is down-regulated in TIF1beta ( HP1box / - ) cells compared with wild-type cells during PrE differentiation .
	manualset3
111422	8	403181	5	NULL	NULL	0	NULL	PrE differentiation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the expression of three endoderm-specific genes , GATA6 , HNF4 , and Dab2 , is down-regulated in TIF1beta ( HP1box / - ) cells compared with wild-type cells during PrE differentiation .
	manualset3
111446	1	403182	5	NULL	NULL	0	NULL	cellular correlate	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A cellular correlate of learning-induced metaplasticity in the hippocampus .
	manualset3
111447	2	403182	5	NULL	NULL	0	NULL	learning-induced metaplasticity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A cellular correlate of learning-induced metaplasticity in the hippocampus .
	manualset3
111448	3	403182	5	NULL	NULL	NULL	NULL	hippocampus 	AnatomicalPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A cellular correlate of learning-induced metaplasticity in the hippocampus .
	manualset3
111449	1	403183	5	NULL	NULL	0	NULL	haplotype -2578 C / -1498 T	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the haplotype -2578 C / -1498 T was less frequent in CRC patients while the -2578 A / -1498 C haplotype was significantly more frequent in patients compared to healthy controls .
	manualset3
111450	2	403183	5	NULL	NULL	0	NULL	CRC patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the haplotype -2578 C / -1498 T was less frequent in CRC patients while the -2578 A / -1498 C haplotype was significantly more frequent in patients compared to healthy controls .
	manualset3
111451	3	403183	5	NULL	NULL	0	NULL	-2578 A / -1498 C haplotype	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the haplotype -2578 C / -1498 T was less frequent in CRC patients while the -2578 A / -1498 C haplotype was significantly more frequent in patients compared to healthy controls .
	manualset3
111452	4	403183	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the haplotype -2578 C / -1498 T was less frequent in CRC patients while the -2578 A / -1498 C haplotype was significantly more frequent in patients compared to healthy controls .
	manualset3
111453	5	403183	5	NULL	NULL	0	NULL	healthy controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the haplotype -2578 C / -1498 T was less frequent in CRC patients while the -2578 A / -1498 C haplotype was significantly more frequent in patients compared to healthy controls .
	manualset3
111454	1	403184	5	NULL	NULL	0	NULL	lack 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the lack of pulmonary hypertension with mefenorex has been demonstrated in both preclinical and clinical studies .
	manualset3
111455	2	403184	5	NULL	NULL	0	NULL	pulmonary hypertension	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the lack of pulmonary hypertension with mefenorex has been demonstrated in both preclinical and clinical studies .
	manualset3
111456	3	403184	5	NULL	NULL	0	NULL	mefenorex 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the lack of pulmonary hypertension with mefenorex has been demonstrated in both preclinical and clinical studies .
	manualset3
111457	4	403184	5	NULL	NULL	0	NULL	preclinical studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the lack of pulmonary hypertension with mefenorex has been demonstrated in both preclinical and clinical studies .
	manualset3
111458	5	403184	5	NULL	NULL	0	NULL	clinical studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the lack of pulmonary hypertension with mefenorex has been demonstrated in both preclinical and clinical studies .
	manualset3
111459	1	403185	5	NULL	NULL	0	NULL	mvp1-1 mutant	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the mvp1-1 mutant showed increased nitrile production during glucosinolate hydrolysis , suggesting that MVP1 may play a role in modulation of myrosinase activity .
	manualset3
111460	2	403185	5	NULL	NULL	0	NULL	nitrile production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the mvp1-1 mutant showed increased nitrile production during glucosinolate hydrolysis , suggesting that MVP1 may play a role in modulation of myrosinase activity .
	manualset3
111461	3	403185	5	NULL	NULL	0	NULL	glucosinolate hydrolysis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the mvp1-1 mutant showed increased nitrile production during glucosinolate hydrolysis , suggesting that MVP1 may play a role in modulation of myrosinase activity .
	manualset3
111462	4	403185	5	NULL	NULL	0	NULL	MVP1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the mvp1-1 mutant showed increased nitrile production during glucosinolate hydrolysis , suggesting that MVP1 may play a role in modulation of myrosinase activity .
	manualset3
111463	5	403185	5	NULL	NULL	0	NULL	play a role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the mvp1-1 mutant showed increased nitrile production during glucosinolate hydrolysis , suggesting that MVP1 may play a role in modulation of myrosinase activity .
	manualset3
111464	6	403185	5	NULL	NULL	0	NULL	modulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the mvp1-1 mutant showed increased nitrile production during glucosinolate hydrolysis , suggesting that MVP1 may play a role in modulation of myrosinase activity .
	manualset3
111465	7	403185	5	NULL	NULL	0	NULL	myrosinase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the mvp1-1 mutant showed increased nitrile production during glucosinolate hydrolysis , suggesting that MVP1 may play a role in modulation of myrosinase activity .
	manualset3
111466	1	403186	5	NULL	NULL	0	NULL	VAP-1 inhibitor	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the new VAP-1 inhibitor effectively prevented the extravasation of PMNs in an animal model of inflammation .
	manualset3
111467	2	403186	5	NULL	NULL	0	NULL	extravasation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the new VAP-1 inhibitor effectively prevented the extravasation of PMNs in an animal model of inflammation .
	manualset3
111468	3	403186	5	NULL	NULL	0	NULL	PMNs 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the new VAP-1 inhibitor effectively prevented the extravasation of PMNs in an animal model of inflammation .
	manualset3
111469	4	403186	5	NULL	NULL	0	NULL	animal model	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the new VAP-1 inhibitor effectively prevented the extravasation of PMNs in an animal model of inflammation .
	manualset3
111470	5	403186	5	NULL	NULL	0	NULL	inflammation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the new VAP-1 inhibitor effectively prevented the extravasation of PMNs in an animal model of inflammation .
	manualset3
111471	1	403187	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the presence of monoacylated PrPC displaced cPLA2 from PrPSc-containing lipid rafts , reducing the activation of cPLA2 and PrPSc formation .
	manualset3
111472	2	403187	5	NULL	NULL	0	NULL	monoacylated PrPC	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the presence of monoacylated PrPC displaced cPLA2 from PrPSc-containing lipid rafts , reducing the activation of cPLA2 and PrPSc formation .
	manualset3
111473	3	403187	5	NULL	NULL	0	NULL	cPLA2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the presence of monoacylated PrPC displaced cPLA2 from PrPSc-containing lipid rafts , reducing the activation of cPLA2 and PrPSc formation .
	manualset3
111474	4	403187	5	NULL	NULL	0	NULL	PrPSc-containing lipid rafts	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the presence of monoacylated PrPC displaced cPLA2 from PrPSc-containing lipid rafts , reducing the activation of cPLA2 and PrPSc formation .
	manualset3
111475	5	403187	5	NULL	NULL	0	NULL	activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the presence of monoacylated PrPC displaced cPLA2 from PrPSc-containing lipid rafts , reducing the activation of cPLA2 and PrPSc formation .
	manualset3
111476	6	403187	5	NULL	NULL	0	NULL	cPLA2 formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the presence of monoacylated PrPC displaced cPLA2 from PrPSc-containing lipid rafts , reducing the activation of cPLA2 and PrPSc formation .
	manualset3
111477	7	403187	5	NULL	NULL	0	NULL	PrPSc formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the presence of monoacylated PrPC displaced cPLA2 from PrPSc-containing lipid rafts , reducing the activation of cPLA2 and PrPSc formation .
	manualset3
111478	1	403188	5	NULL	NULL	NULL	NULL	rank-order	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Moreover , the rank-order of substrate cutting is similar in apoptotic cells , suggesting that cellular structures do not dramatically alter substrate accessibility .
	manualset3
111479	2	403188	5	NULL	NULL	0	NULL	substrate cutting	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the rank-order of substrate cutting is similar in apoptotic cells , suggesting that cellular structures do not dramatically alter substrate accessibility .
	manualset3
111480	3	403188	5	NULL	NULL	0	NULL	apoptotic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the rank-order of substrate cutting is similar in apoptotic cells , suggesting that cellular structures do not dramatically alter substrate accessibility .
	manualset3
111481	4	403188	5	NULL	NULL	0	NULL	cellular structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the rank-order of substrate cutting is similar in apoptotic cells , suggesting that cellular structures do not dramatically alter substrate accessibility .
	manualset3
111482	5	403188	5	NULL	NULL	0	NULL	substrate accessibility	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the rank-order of substrate cutting is similar in apoptotic cells , suggesting that cellular structures do not dramatically alter substrate accessibility .
	manualset3
111483	1	403189	5	NULL	NULL	0	NULL	reported case	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the reported case recalls the need to strengthen the collaboration between the cardiologist and the occupational health physician .
	manualset3
111484	2	403189	5	NULL	NULL	0	NULL	collaboration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the reported case recalls the need to strengthen the collaboration between the cardiologist and the occupational health physician .
	manualset3
111485	3	403189	5	NULL	NULL	0	NULL	cardiologist 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the reported case recalls the need to strengthen the collaboration between the cardiologist and the occupational health physician .
	manualset3
111486	4	403189	5	NULL	NULL	0	NULL	occupational health physician	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the reported case recalls the need to strengthen the collaboration between the cardiologist and the occupational health physician .
	manualset3
111487	1	403190	5	NULL	NULL	0	NULL	retinoid content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the retinoid content and the effects of RA treatment have been described in a number of invertebrates , although the physiological role of RA signaling outside vertebrates is still not fully understood .
	manualset3
111488	2	403190	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the retinoid content and the effects of RA treatment have been described in a number of invertebrates , although the physiological role of RA signaling outside vertebrates is still not fully understood .
	manualset3
111489	3	403190	5	NULL	NULL	NULL	NULL	RA treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Moreover , the retinoid content and the effects of RA treatment have been described in a number of invertebrates , although the physiological role of RA signaling outside vertebrates is still not fully understood .
	manualset3
111490	4	403190	5	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the retinoid content and the effects of RA treatment have been described in a number of invertebrates , although the physiological role of RA signaling outside vertebrates is still not fully understood .
	manualset3
111491	5	403190	5	NULL	NULL	0	NULL	invertebrates 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the retinoid content and the effects of RA treatment have been described in a number of invertebrates , although the physiological role of RA signaling outside vertebrates is still not fully understood .
	manualset3
111492	6	403190	5	NULL	NULL	0	NULL	physiological role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the retinoid content and the effects of RA treatment have been described in a number of invertebrates , although the physiological role of RA signaling outside vertebrates is still not fully understood .
	manualset3
111493	7	403190	5	NULL	NULL	0	NULL	RA signaling 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the retinoid content and the effects of RA treatment have been described in a number of invertebrates , although the physiological role of RA signaling outside vertebrates is still not fully understood .
	manualset3
111494	8	403190	5	NULL	NULL	0	NULL	vertebrates 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the retinoid content and the effects of RA treatment have been described in a number of invertebrates , although the physiological role of RA signaling outside vertebrates is still not fully understood .
	manualset3
111495	1	403191	5	NULL	NULL	0	NULL	takovite catalyst	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the takovite catalyst was found to be stable under reaction conditions and recyclable .
	manualset3
111496	2	403191	5	NULL	NULL	0	NULL	reaction conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the takovite catalyst was found to be stable under reaction conditions and recyclable .
	manualset3
111497	1	403192	5	NULL	NULL	0	NULL	test 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the test was successfully evaluated on 10 atypical S. pneumoniae strains related to pneumococcal diseases .
	manualset3
111498	2	403192	5	NULL	NULL	NULL	NULL	10 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Moreover , the test was successfully evaluated on 10 atypical S. pneumoniae strains related to pneumococcal diseases .
	manualset3
111499	4	403192	5	NULL	NULL	NULL	NULL	pneumococcal diseases	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Moreover , the test was successfully evaluated on 10 atypical S. pneumoniae strains related to pneumococcal diseases .
	manualset3
112979	3	403192	5	NULL	NULL	0	NULL	atypicaS. pneumoniae strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the test was successfully evaluated on 10 atypical S. pneumoniae strains related to pneumococcal diseases .
	manualset3
111500	1	403193	5	NULL	NULL	0	NULL	central difficulty 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A central difficulty of brain modelling is to span the range of spatio-temporal scales from synapses to the whole brain .
	manualset3
111501	2	403193	5	NULL	NULL	0	NULL	brain modelling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A central difficulty of brain modelling is to span the range of spatio-temporal scales from synapses to the whole brain .
	manualset3
111503	4	403193	5	NULL	NULL	0	NULL	range 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A central difficulty of brain modelling is to span the range of spatio-temporal scales from synapses to the whole brain .
	manualset3
111504	5	403193	5	NULL	NULL	0	NULL	spatio-temporal scales	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A central difficulty of brain modelling is to span the range of spatio-temporal scales from synapses to the whole brain .
	manualset3
111505	6	403193	5	NULL	NULL	0	NULL	synapses 	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A central difficulty of brain modelling is to span the range of spatio-temporal scales from synapses to the whole brain .
	manualset3
111506	7	403193	5	NULL	NULL	0	NULL	whole brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A central difficulty of brain modelling is to span the range of spatio-temporal scales from synapses to the whole brain .
	manualset3
111507	1	403194	5	NULL	NULL	0	NULL	three-dimensional potential energy surface	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the three-dimensional potential energy surface also shows that the previously proposed pathway , involving Glu166 as the general base promoting Ser70 through a conserved water molecule , exists in competition with the Lys73 process .
	manualset3
111508	2	403194	5	NULL	NULL	0	NULL	previously proposed pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the three-dimensional potential energy surface also shows that the previously proposed pathway , involving Glu166 as the general base promoting Ser70 through a conserved water molecule , exists in competition with the Lys73 process .
	manualset3
111509	3	403194	5	NULL	NULL	0	NULL	Glu166 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the three-dimensional potential energy surface also shows that the previously proposed pathway , involving Glu166 as the general base promoting Ser70 through a conserved water molecule , exists in competition with the Lys73 process .
	manualset3
111510	4	403194	5	NULL	NULL	0	NULL	general base	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the three-dimensional potential energy surface also shows that the previously proposed pathway , involving Glu166 as the general base promoting Ser70 through a conserved water molecule , exists in competition with the Lys73 process .
	manualset3
111511	5	403194	5	NULL	NULL	0	NULL	Ser70	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the three-dimensional potential energy surface also shows that the previously proposed pathway , involving Glu166 as the general base promoting Ser70 through a conserved water molecule , exists in competition with the Lys73 process .
	manualset3
111512	6	403194	5	NULL	NULL	0	NULL	conserved water molecule 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the three-dimensional potential energy surface also shows that the previously proposed pathway , involving Glu166 as the general base promoting Ser70 through a conserved water molecule , exists in competition with the Lys73 process .
	manualset3
111513	7	403194	5	NULL	NULL	0	NULL	competition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the three-dimensional potential energy surface also shows that the previously proposed pathway , involving Glu166 as the general base promoting Ser70 through a conserved water molecule , exists in competition with the Lys73 process .
	manualset3
111514	8	403194	5	NULL	NULL	0	NULL	Lys73 process	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the three-dimensional potential energy surface also shows that the previously proposed pathway , involving Glu166 as the general base promoting Ser70 through a conserved water molecule , exists in competition with the Lys73 process .
	manualset3
111515	1	403195	5	NULL	NULL	0	NULL	time interval	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the time interval between attempts to impregnate and obtainment of pregnancy was correlated ( P less than 0.01 ) .
	manualset3
111516	2	403195	5	NULL	NULL	0	NULL	attempts 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the time interval between attempts to impregnate and obtainment of pregnancy was correlated ( P less than 0.01 ) .
	manualset3
111517	3	403195	5	NULL	NULL	0	NULL	obtainment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the time interval between attempts to impregnate and obtainment of pregnancy was correlated ( P less than 0.01 ) .
	manualset3
111518	4	403195	5	NULL	NULL	0	NULL	pregnancy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the time interval between attempts to impregnate and obtainment of pregnancy was correlated ( P less than 0.01 ) .
	manualset3
111519	5	403195	5	NULL	NULL	0	NULL	P less than 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the time interval between attempts to impregnate and obtainment of pregnancy was correlated ( P less than 0.01 ) .
	manualset3
111520	1	403196	5	NULL	NULL	0	NULL	proliferative activity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , there was decreased proliferative activity with downregulation of Flk-1 in tumor cells isolated from conditional knockout ( VEGF ( - / - ) ) MT-induced mammary carcinomas .
	manualset3
111521	2	403196	5	NULL	NULL	0	NULL	downregulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , there was decreased proliferative activity with downregulation of Flk-1 in tumor cells isolated from conditional knockout ( VEGF ( - / - ) ) MT-induced mammary carcinomas .
	manualset3
111522	3	403196	5	NULL	NULL	0	NULL	Flk-1	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , there was decreased proliferative activity with downregulation of Flk-1 in tumor cells isolated from conditional knockout ( VEGF ( - / - ) ) MT-induced mammary carcinomas .
	manualset3
111523	4	403196	5	NULL	NULL	0	NULL	tumor cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , there was decreased proliferative activity with downregulation of Flk-1 in tumor cells isolated from conditional knockout ( VEGF ( - / - ) ) MT-induced mammary carcinomas .
	manualset3
111524	5	403196	5	NULL	NULL	0	NULL	conditional knockout ( VEGF ( - / - ) ) MT-induced mammary carcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , there was decreased proliferative activity with downregulation of Flk-1 in tumor cells isolated from conditional knockout ( VEGF ( - / - ) ) MT-induced mammary carcinomas .
	manualset3
111525	1	403197	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , these results also suggest that the propagation of the Ca2 + - activated and Gi3-mediated signaling pathway requires the blocking of Gi3 GTPase activity .
	manualset3
111526	2	403197	5	NULL	NULL	0	NULL	propagation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , these results also suggest that the propagation of the Ca2 + - activated and Gi3-mediated signaling pathway requires the blocking of Gi3 GTPase activity .
	manualset3
111527	3	403197	5	NULL	NULL	0	NULL	Ca2 + - activated signaling pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , these results also suggest that the propagation of the Ca2 + - activated and Gi3-mediated signaling pathway requires the blocking of Gi3 GTPase activity .
	manualset3
111528	4	403197	5	NULL	NULL	0	NULL	Gi3-mediated signaling pathway 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , these results also suggest that the propagation of the Ca2 + - activated and Gi3-mediated signaling pathway requires the blocking of Gi3 GTPase activity .
	manualset3
111529	5	403197	5	NULL	NULL	0	NULL	Gi3 GTPase activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , these results also suggest that the propagation of the Ca2 + - activated and Gi3-mediated signaling pathway requires the blocking of Gi3 GTPase activity .
	manualset3
111530	1	403198	5	NULL	NULL	0	NULL	proposed mechanisms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , these two proposed mechanisms of EGCG-induced cell proliferation may differ kinetically to promote keratinocyte survival .
	manualset3
111592	2	403198	5	NULL	NULL	0	NULL	EGCG-induced cell proliferation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , these two proposed mechanisms of EGCG-induced cell proliferation may differ kinetically to promote keratinocyte survival .
	manualset3
111593	3	403198	5	NULL	NULL	NULL	NULL	keratinocyte survival	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Moreover , these two proposed mechanisms of EGCG-induced cell proliferation may differ kinetically to promote keratinocyte survival .
	manualset3
111594	1	403199	5	NULL	NULL	0	NULL	combination augmented antitumor activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , this combination augmented antitumor activity against murine S180 and M109 tumors , and human LX-1 and LS180 tumor xenografts in mice .
	manualset3
111595	2	403199	5	NULL	NULL	0	NULL	murine S180 tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , this combination augmented antitumor activity against murine S180 and M109 tumors , and human LX-1 and LS180 tumor xenografts in mice .
	manualset3
111596	3	403199	5	NULL	NULL	0	NULL	murine M109 tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , this combination augmented antitumor activity against murine S180 and M109 tumors , and human LX-1 and LS180 tumor xenografts in mice .
	manualset3
111597	4	403199	5	NULL	NULL	NULL	NULL	human LX-1 tumor xenograft	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Moreover , this combination augmented antitumor activity against murine S180 and M109 tumors , and human LX-1 and LS180 tumor xenografts in mice .
	manualset3
111598	5	403199	5	NULL	NULL	NULL	NULL	human LS180 tumor xenografts 	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Moreover , this combination augmented antitumor activity against murine S180 and M109 tumors , and human LX-1 and LS180 tumor xenografts in mice .
	manualset3
111599	6	403199	5	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , this combination augmented antitumor activity against murine S180 and M109 tumors , and human LX-1 and LS180 tumor xenografts in mice .
	manualset3
111600	1	403200	5	NULL	NULL	NULL	NULL	presence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Moreover , this decrease was not observed in the presence of cycloheximide , and a closely comparable amount of the primary transcripts was detected in both Had-2 and FM3A cells .
	manualset3
111601	2	403200	5	NULL	NULL	0	NULL	cycloheximide	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , this decrease was not observed in the presence of cycloheximide , and a closely comparable amount of the primary transcripts was detected in both Had-2 and FM3A cells .
	manualset3
111602	3	403200	5	NULL	NULL	0	NULL	closely comparable amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , this decrease was not observed in the presence of cycloheximide , and a closely comparable amount of the primary transcripts was detected in both Had-2 and FM3A cells .
	manualset3
111603	4	403200	5	NULL	NULL	0	NULL	primary transcripts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , this decrease was not observed in the presence of cycloheximide , and a closely comparable amount of the primary transcripts was detected in both Had-2 and FM3A cells .
	manualset3
111604	5	403200	5	NULL	NULL	0	NULL	Had-2 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , this decrease was not observed in the presence of cycloheximide , and a closely comparable amount of the primary transcripts was detected in both Had-2 and FM3A cells .
	manualset3
111605	6	403200	5	NULL	NULL	0	NULL	FM3A cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , this decrease was not observed in the presence of cycloheximide , and a closely comparable amount of the primary transcripts was detected in both Had-2 and FM3A cells .
	manualset3
111606	1	403201	5	NULL	NULL	0	NULL	tryptic on-target digestion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , tryptic on-target digestion of the collected protein fractions , with subsequent MALDI-MS and MS/MS peptide analysis , was demonstrated .
	manualset3
111607	2	403201	5	NULL	NULL	0	NULL	collected protein fractions	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , tryptic on-target digestion of the collected protein fractions , with subsequent MALDI-MS and MS/MS peptide analysis , was demonstrated .
	manualset3
111608	3	403201	5	NULL	NULL	0	NULL	MALDI-MS	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , tryptic on-target digestion of the collected protein fractions , with subsequent MALDI-MS and MS/MS peptide analysis , was demonstrated .
	manualset3
111609	4	403201	5	NULL	NULL	0	NULL	MS/MS peptide analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , tryptic on-target digestion of the collected protein fractions , with subsequent MALDI-MS and MS/MS peptide analysis , was demonstrated .
	manualset3
111610	1	403202	5	NULL	NULL	0	NULL	velar lowering	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , velar lowering for the nasal consonant began in close temporal proximity to the nasal murmur .
	manualset3
111611	2	403202	5	NULL	NULL	0	NULL	nasal consonant	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , velar lowering for the nasal consonant began in close temporal proximity to the nasal murmur .
	manualset3
111613	3	403202	5	NULL	NULL	0	NULL	temporal proximity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , velar lowering for the nasal consonant began in close temporal proximity to the nasal murmur .
	manualset3
111614	4	403202	5	NULL	NULL	0	NULL	nasal murmur	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , velar lowering for the nasal consonant began in close temporal proximity to the nasal murmur .
	manualset3
111615	1	403203	5	NULL	NULL	0	NULL	VEGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we demonstrate that VEGF in CRCC tumors is mainly produced by tumor stromal cells instead of the tumor cells themselves .
	manualset3
111616	2	403203	5	NULL	NULL	0	NULL	CRCC tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we demonstrate that VEGF in CRCC tumors is mainly produced by tumor stromal cells instead of the tumor cells themselves .
	manualset3
111617	3	403203	5	NULL	NULL	0	NULL	tumor stromal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we demonstrate that VEGF in CRCC tumors is mainly produced by tumor stromal cells instead of the tumor cells themselves .
	manualset3
111618	4	403203	5	NULL	NULL	0	NULL	tumor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we demonstrate that VEGF in CRCC tumors is mainly produced by tumor stromal cells instead of the tumor cells themselves .
	manualset3
111619	1	403204	5	NULL	NULL	0	NULL	simple procedure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we develop a simple procedure for increased efficiency of the algorithm .
	manualset3
111620	2	403204	5	NULL	NULL	0	NULL	increased efficiency	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we develop a simple procedure for increased efficiency of the algorithm .
	manualset3
111621	3	403204	5	NULL	NULL	0	NULL	algorithm	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we develop a simple procedure for increased efficiency of the algorithm .
	manualset3
111622	1	403205	5	NULL	NULL	0	NULL	MDC1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we establish that MDC1 recruits RNF8 through phosphodependent interactions between the RNF8 forkhead-associated domain and motifs in MDC1 that are phosphorylated by the DNA-damage activated protein kinase ataxia telangiectasia mutated ( ATM ) .
	manualset3
111623	2	403205	5	NULL	NULL	0	NULL	RNF8	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we establish that MDC1 recruits RNF8 through phosphodependent interactions between the RNF8 forkhead-associated domain and motifs in MDC1 that are phosphorylated by the DNA-damage activated protein kinase ataxia telangiectasia mutated ( ATM ) .
	manualset3
111624	3	403205	5	NULL	NULL	0	NULL	phosphodependent interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we establish that MDC1 recruits RNF8 through phosphodependent interactions between the RNF8 forkhead-associated domain and motifs in MDC1 that are phosphorylated by the DNA-damage activated protein kinase ataxia telangiectasia mutated ( ATM ) .
	manualset3
111625	4	403205	5	NULL	NULL	0	NULL	RNF8 forkhead-associated domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we establish that MDC1 recruits RNF8 through phosphodependent interactions between the RNF8 forkhead-associated domain and motifs in MDC1 that are phosphorylated by the DNA-damage activated protein kinase ataxia telangiectasia mutated ( ATM ) .
	manualset3
111626	5	403205	5	NULL	NULL	0	NULL	MDC1 motifs	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we establish that MDC1 recruits RNF8 through phosphodependent interactions between the RNF8 forkhead-associated domain and motifs in MDC1 that are phosphorylated by the DNA-damage activated protein kinase ataxia telangiectasia mutated ( ATM ) .
	manualset3
111627	6	403205	5	NULL	NULL	0	NULL	 DNA-damage activated protein kinase ataxia telangiectasia mutated ( ATM )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we establish that MDC1 recruits RNF8 through phosphodependent interactions between the RNF8 forkhead-associated domain and motifs in MDC1 that are phosphorylated by the DNA-damage activated protein kinase ataxia telangiectasia mutated ( ATM ) .
	manualset3
111628	1	403206	5	NULL	NULL	0	NULL	previously developed methods 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we use our previously developed methods to calculate the relaxation of the C-H stretch mode via vibration-phonon interaction , using the Born-Oppenheimer surface for all local modes as obtained from the DFT calculations .
	manualset3
111629	2	403206	5	NULL	NULL	0	NULL	calculate	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we use our previously developed methods to calculate the relaxation of the C-H stretch mode via vibration-phonon interaction , using the Born-Oppenheimer surface for all local modes as obtained from the DFT calculations .
	manualset3
111630	3	403206	5	NULL	NULL	0	NULL	relaxation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we use our previously developed methods to calculate the relaxation of the C-H stretch mode via vibration-phonon interaction , using the Born-Oppenheimer surface for all local modes as obtained from the DFT calculations .
	manualset3
111631	4	403206	5	NULL	NULL	0	NULL	C-H stretch mode	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we use our previously developed methods to calculate the relaxation of the C-H stretch mode via vibration-phonon interaction , using the Born-Oppenheimer surface for all local modes as obtained from the DFT calculations .
	manualset3
111632	5	403206	5	NULL	NULL	0	NULL	vibration-phonon interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we use our previously developed methods to calculate the relaxation of the C-H stretch mode via vibration-phonon interaction , using the Born-Oppenheimer surface for all local modes as obtained from the DFT calculations .
	manualset3
111633	6	403206	5	NULL	NULL	0	NULL	Born-Oppenheimer surface	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we use our previously developed methods to calculate the relaxation of the C-H stretch mode via vibration-phonon interaction , using the Born-Oppenheimer surface for all local modes as obtained from the DFT calculations .
	manualset3
111634	7	403206	5	NULL	NULL	0	NULL	local modes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we use our previously developed methods to calculate the relaxation of the C-H stretch mode via vibration-phonon interaction , using the Born-Oppenheimer surface for all local modes as obtained from the DFT calculations .
	manualset3
111635	8	403206	5	NULL	NULL	0	NULL	DFT calculations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we use our previously developed methods to calculate the relaxation of the C-H stretch mode via vibration-phonon interaction , using the Born-Oppenheimer surface for all local modes as obtained from the DFT calculations .
	manualset3
111636	1	403207	5	NULL	NULL	0	NULL	western R. pomonella	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , western R. pomonella display both positive orientation to their respective natal fruit volatiles and avoidance behavior ( negative orientation ) to non-natal volatiles .
	manualset3
111637	2	403207	5	NULL	NULL	0	NULL	positive orientation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , western R. pomonella display both positive orientation to their respective natal fruit volatiles and avoidance behavior ( negative orientation ) to non-natal volatiles .
	manualset3
111639	3	403207	5	NULL	NULL	0	NULL	natal fruit volatiles	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , western R. pomonella display both positive orientation to their respective natal fruit volatiles and avoidance behavior ( negative orientation ) to non-natal volatiles .
	manualset3
111661	4	403207	5	NULL	NULL	0	NULL	avoidance behavior ( negative orientation )	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , western R. pomonella display both positive orientation to their respective natal fruit volatiles and avoidance behavior ( negative orientation ) to non-natal volatiles .
	manualset3
111662	5	403207	5	NULL	NULL	0	NULL	non-natal volatiles	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , western R. pomonella display both positive orientation to their respective natal fruit volatiles and avoidance behavior ( negative orientation ) to non-natal volatiles .
	manualset3
111663	1	403208	5	NULL	NULL	0	NULL	functional heterogeneity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover functional heterogeneity of islets is suggested .
	manualset3
111664	2	403208	5	NULL	NULL	0	NULL	islets	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover functional heterogeneity of islets is suggested .
	manualset3
111715	1	403209	5	NULL	NULL	0	NULL	chequered life	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A chequered life -- Eugene SUE ( 1804-1857 ) , physician and novelist .
	manualset3
111716	2	403209	5	NULL	NULL	0	NULL	Eugene SUE	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A chequered life -- Eugene SUE ( 1804-1857 ) , physician and novelist .
	manualset3
111717	3	403209	5	NULL	NULL	0	NULL	1804-1857	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A chequered life -- Eugene SUE ( 1804-1857 ) , physician and novelist .
	manualset3
111718	4	403209	5	NULL	NULL	0	NULL	physician	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A chequered life -- Eugene SUE ( 1804-1857 ) , physician and novelist .
	manualset3
111719	5	403209	5	NULL	NULL	0	NULL	novelist	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A chequered life -- Eugene SUE ( 1804-1857 ) , physician and novelist .
	manualset3
111720	1	403210	5	NULL	NULL	NULL	NULL	Morphine dependence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Morphine dependence intensified splenocyte infiltration into the CNS following neuroinflammation induced by IFN - gene transfer .
	manualset3
111721	2	403210	5	NULL	NULL	0	NULL	splenocyte infiltration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphine dependence intensified splenocyte infiltration into the CNS following neuroinflammation induced by IFN - gene transfer .
	manualset3
111722	3	403210	5	NULL	NULL	0	NULL	CNS	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphine dependence intensified splenocyte infiltration into the CNS following neuroinflammation induced by IFN - gene transfer .
	manualset3
111723	4	403210	5	NULL	NULL	0	NULL	neuroinflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphine dependence intensified splenocyte infiltration into the CNS following neuroinflammation induced by IFN - gene transfer .
	manualset3
111724	5	403210	5	NULL	NULL	0	NULL	IFN - gene transfer 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphine dependence intensified splenocyte infiltration into the CNS following neuroinflammation induced by IFN - gene transfer .
	manualset3
111725	1	403211	5	NULL	NULL	0	NULL	Morphine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphine is now said to have no problematic side effects such as analgesic tolerance and physical dependence for cancer pain patients in clinic , as far as it is appropriately used .
	manualset3
111726	2	403211	5	NULL	NULL	0	NULL	problematic side effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphine is now said to have no problematic side effects such as analgesic tolerance and physical dependence for cancer pain patients in clinic , as far as it is appropriately used .
	manualset3
111727	3	403211	5	NULL	NULL	0	NULL	analgesic tolerance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphine is now said to have no problematic side effects such as analgesic tolerance and physical dependence for cancer pain patients in clinic , as far as it is appropriately used .
	manualset3
111728	4	403211	5	NULL	NULL	0	NULL	physical dependence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphine is now said to have no problematic side effects such as analgesic tolerance and physical dependence for cancer pain patients in clinic , as far as it is appropriately used .
	manualset3
111729	5	403211	5	NULL	NULL	0	NULL	cancer pain patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphine is now said to have no problematic side effects such as analgesic tolerance and physical dependence for cancer pain patients in clinic , as far as it is appropriately used .
	manualset3
111730	6	403211	5	NULL	NULL	0	NULL	clinic	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphine is now said to have no problematic side effects such as analgesic tolerance and physical dependence for cancer pain patients in clinic , as far as it is appropriately used .
	manualset3
111731	1	403212	5	NULL	NULL	0	NULL	Morphologic features	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphologic features of the myopathy associated with chronic renal failure .
	manualset3
111732	2	403212	5	NULL	NULL	0	NULL	myopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphologic features of the myopathy associated with chronic renal failure .
	manualset3
111733	3	403212	5	NULL	NULL	0	NULL	chronic renal failure	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphologic features of the myopathy associated with chronic renal failure .
	manualset3
111734	1	403213	5	NULL	NULL	0	NULL	Morphological analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphological analysis of parasite development proved a sensitive assay , since development of mature trophozoites was inhibited 50 % by 25 microM 2-F-HIS or 100 2-I-HIS .
	manualset3
111735	2	403213	5	NULL	NULL	0	NULL	parasite development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphological analysis of parasite development proved a sensitive assay , since development of mature trophozoites was inhibited 50 % by 25 microM 2-F-HIS or 100 2-I-HIS .
	manualset3
111736	3	403213	5	NULL	NULL	0	NULL	sensitive assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphological analysis of parasite development proved a sensitive assay , since development of mature trophozoites was inhibited 50 % by 25 microM 2-F-HIS or 100 2-I-HIS .
	manualset3
111870	4	403213	5	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphological analysis of parasite development proved a sensitive assay , since development of mature trophozoites was inhibited 50 % by 25 microM 2-F-HIS or 100 2-I-HIS .
	manualset3
111871	5	403213	5	NULL	NULL	0	NULL	mature trophozoites	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphological analysis of parasite development proved a sensitive assay , since development of mature trophozoites was inhibited 50 % by 25 microM 2-F-HIS or 100 2-I-HIS .
	manualset3
111872	6	403213	5	NULL	NULL	0	NULL	50 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphological analysis of parasite development proved a sensitive assay , since development of mature trophozoites was inhibited 50 % by 25 microM 2-F-HIS or 100 2-I-HIS .
	manualset3
111873	7	403213	5	NULL	NULL	0	NULL	25 microM 2-F-HIS	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphological analysis of parasite development proved a sensitive assay , since development of mature trophozoites was inhibited 50 % by 25 microM 2-F-HIS or 100 2-I-HIS .
	manualset3
111874	8	403213	5	NULL	NULL	0	NULL	100 2-I-HIS	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphological analysis of parasite development proved a sensitive assay , since development of mature trophozoites was inhibited 50 % by 25 microM 2-F-HIS or 100 2-I-HIS .
	manualset3
111875	1	403214	5	NULL	NULL	0	NULL	Morphological evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphological evaluation of the cells treated with UV radiation showed an increase in degeneration of chromatin and a decrease in cell size as compared to non-treated groups .
	manualset3
111876	2	403214	5	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphological evaluation of the cells treated with UV radiation showed an increase in degeneration of chromatin and a decrease in cell size as compared to non-treated groups .
	manualset3
111877	3	403214	5	NULL	NULL	0	NULL	UV radiation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphological evaluation of the cells treated with UV radiation showed an increase in degeneration of chromatin and a decrease in cell size as compared to non-treated groups .
	manualset3
111878	4	403214	5	NULL	NULL	0	NULL	degeneration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphological evaluation of the cells treated with UV radiation showed an increase in degeneration of chromatin and a decrease in cell size as compared to non-treated groups .
	manualset3
111879	5	403214	5	NULL	NULL	0	NULL	chromatin	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphological evaluation of the cells treated with UV radiation showed an increase in degeneration of chromatin and a decrease in cell size as compared to non-treated groups .
	manualset3
111880	6	403214	5	NULL	NULL	0	NULL	cell size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphological evaluation of the cells treated with UV radiation showed an increase in degeneration of chromatin and a decrease in cell size as compared to non-treated groups .
	manualset3
111881	7	403214	5	NULL	NULL	0	NULL	non-treated groups	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphological evaluation of the cells treated with UV radiation showed an increase in degeneration of chromatin and a decrease in cell size as compared to non-treated groups .
	manualset3
111882	1	403215	5	NULL	NULL	0	NULL	Morphological examination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphological examination of the lymph nodes with undifferentiated carcinoma metastasis from 52 patients without an identified primary tumor at the time of biopsy has been performed .
	manualset3
111883	2	403215	5	NULL	NULL	0	NULL	lymph nodes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphological examination of the lymph nodes with undifferentiated carcinoma metastasis from 52 patients without an identified primary tumor at the time of biopsy has been performed .
	manualset3
111884	3	403215	5	NULL	NULL	0	NULL	undifferentiated carcinoma metastasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphological examination of the lymph nodes with undifferentiated carcinoma metastasis from 52 patients without an identified primary tumor at the time of biopsy has been performed .
	manualset3
111885	4	403215	5	NULL	NULL	NULL	NULL	52 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Morphological examination of the lymph nodes with undifferentiated carcinoma metastasis from 52 patients without an identified primary tumor at the time of biopsy has been performed .
	manualset3
111886	6	403215	5	NULL	NULL	NULL	NULL	primary tumor 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Morphological examination of the lymph nodes with undifferentiated carcinoma metastasis from 52 patients without an identified primary tumor at the time of biopsy has been performed .
	manualset3
111887	7	403215	5	NULL	NULL	NULL	NULL	time	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Morphological examination of the lymph nodes with undifferentiated carcinoma metastasis from 52 patients without an identified primary tumor at the time of biopsy has been performed .
	manualset3
111888	8	403215	5	NULL	NULL	NULL	NULL	biopsy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Morphological examination of the lymph nodes with undifferentiated carcinoma metastasis from 52 patients without an identified primary tumor at the time of biopsy has been performed .
	manualset3
112980	5	403215	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphological examination of the lymph nodes with undifferentiated carcinoma metastasis from 52 patients without an identified primary tumor at the time of biopsy has been performed .
	manualset3
111889	1	403216	5	NULL	NULL	0	NULL	Morphological features	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphological features that separate these taxa from Halophytophthora are a smaller hyphal diameter , oospore production , lack of vesicle formation during sporulation , and a plug of hyaline material at the sporangial apex that is displaced during zoospore release .
	manualset3
111908	2	403216	5	NULL	NULL	0	NULL	taxa 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphological features that separate these taxa from Halophytophthora are a smaller hyphal diameter , oospore production , lack of vesicle formation during sporulation , and a plug of hyaline material at the sporangial apex that is displaced during zoospore release .
	manualset3
111909	3	403216	5	NULL	NULL	0	NULL	Halophytophthora 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphological features that separate these taxa from Halophytophthora are a smaller hyphal diameter , oospore production , lack of vesicle formation during sporulation , and a plug of hyaline material at the sporangial apex that is displaced during zoospore release .
	manualset3
111910	4	403216	5	NULL	NULL	0	NULL	hyphal diameter	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphological features that separate these taxa from Halophytophthora are a smaller hyphal diameter , oospore production , lack of vesicle formation during sporulation , and a plug of hyaline material at the sporangial apex that is displaced during zoospore release .
	manualset3
111911	5	403216	5	NULL	NULL	0	NULL	oospore production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphological features that separate these taxa from Halophytophthora are a smaller hyphal diameter , oospore production , lack of vesicle formation during sporulation , and a plug of hyaline material at the sporangial apex that is displaced during zoospore release .
	manualset3
111912	6	403216	5	NULL	NULL	0	NULL	vesicle formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphological features that separate these taxa from Halophytophthora are a smaller hyphal diameter , oospore production , lack of vesicle formation during sporulation , and a plug of hyaline material at the sporangial apex that is displaced during zoospore release .
	manualset3
111913	7	403216	5	NULL	NULL	0	NULL	sporulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphological features that separate these taxa from Halophytophthora are a smaller hyphal diameter , oospore production , lack of vesicle formation during sporulation , and a plug of hyaline material at the sporangial apex that is displaced during zoospore release .
	manualset3
111914	8	403216	5	NULL	NULL	0	NULL	plug of hyaline material	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphological features that separate these taxa from Halophytophthora are a smaller hyphal diameter , oospore production , lack of vesicle formation during sporulation , and a plug of hyaline material at the sporangial apex that is displaced during zoospore release .
	manualset3
111915	9	403216	5	NULL	NULL	0	NULL	sporangial apex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphological features that separate these taxa from Halophytophthora are a smaller hyphal diameter , oospore production , lack of vesicle formation during sporulation , and a plug of hyaline material at the sporangial apex that is displaced during zoospore release .
	manualset3
111916	10	403216	5	NULL	NULL	0	NULL	zoospore release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphological features that separate these taxa from Halophytophthora are a smaller hyphal diameter , oospore production , lack of vesicle formation during sporulation , and a plug of hyaline material at the sporangial apex that is displaced during zoospore release .
	manualset3
111917	1	403217	5	NULL	NULL	NULL	NULL	Morphologically heterogeneous met-enkephalin terminals	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Morphologically heterogeneous met-enkephalin terminals form synapses with tyrosine hydroxylase-containing dendrites in the rat nucleus locus coeruleus .
	manualset3
111918	2	403217	5	NULL	NULL	0	NULL	synapses 	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphologically heterogeneous met-enkephalin terminals form synapses with tyrosine hydroxylase-containing dendrites in the rat nucleus locus coeruleus .
	manualset3
111919	3	403217	5	NULL	NULL	NULL	NULL	tyrosine hydroxylase-containing dendrites	AnatomicalPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Morphologically heterogeneous met-enkephalin terminals form synapses with tyrosine hydroxylase-containing dendrites in the rat nucleus locus coeruleus .
	manualset3
111920	4	403217	5	NULL	NULL	0	NULL	rat nucleus locus coeruleus	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphologically heterogeneous met-enkephalin terminals form synapses with tyrosine hydroxylase-containing dendrites in the rat nucleus locus coeruleus .
	manualset3
111921	1	403218	5	NULL	NULL	0	NULL	Morphology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphology , electrophysiology and functional input connectivity of pyramidal neurons characterizes a genuine layer va in the primary somatosensory cortex .
	manualset3
111922	2	403218	5	NULL	NULL	0	NULL	electrophysiology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphology , electrophysiology and functional input connectivity of pyramidal neurons characterizes a genuine layer va in the primary somatosensory cortex .
	manualset3
111923	3	403218	5	NULL	NULL	0	NULL	functional input connectivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphology , electrophysiology and functional input connectivity of pyramidal neurons characterizes a genuine layer va in the primary somatosensory cortex .
	manualset3
111924	4	403218	5	NULL	NULL	0	NULL	pyramidal neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphology , electrophysiology and functional input connectivity of pyramidal neurons characterizes a genuine layer va in the primary somatosensory cortex .
	manualset3
111925	5	403218	5	NULL	NULL	0	NULL	genuine layer	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphology , electrophysiology and functional input connectivity of pyramidal neurons characterizes a genuine layer va in the primary somatosensory cortex .
	manualset3
111926	6	403218	5	NULL	NULL	0	NULL	primary somatosensory cortex	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphology , electrophysiology and functional input connectivity of pyramidal neurons characterizes a genuine layer va in the primary somatosensory cortex .
	manualset3
111927	1	403219	5	NULL	NULL	0	NULL	Morphology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphology and surface profiles of the electrodes examined by reflected light , electron , and atomic force microscopy were consistent with those of corrosion resistance , showing that the electrodes with higher corrosion resistance had lower surface roughness than others .
	manualset3
111928	2	403219	5	NULL	NULL	0	NULL	surface profiles	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphology and surface profiles of the electrodes examined by reflected light , electron , and atomic force microscopy were consistent with those of corrosion resistance , showing that the electrodes with higher corrosion resistance had lower surface roughness than others .
	manualset3
111929	3	403219	5	NULL	NULL	0	NULL	electrodes 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphology and surface profiles of the electrodes examined by reflected light , electron , and atomic force microscopy were consistent with those of corrosion resistance , showing that the electrodes with higher corrosion resistance had lower surface roughness than others .
	manualset3
111930	4	403219	5	NULL	NULL	0	NULL	reflected light , electron , and atomic force microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphology and surface profiles of the electrodes examined by reflected light , electron , and atomic force microscopy were consistent with those of corrosion resistance , showing that the electrodes with higher corrosion resistance had lower surface roughness than others .
	manualset3
111931	5	403219	5	NULL	NULL	NULL	NULL	corrosion resistance	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Morphology and surface profiles of the electrodes examined by reflected light , electron , and atomic force microscopy were consistent with those of corrosion resistance , showing that the electrodes with higher corrosion resistance had lower surface roughness than others .
	manualset3
111932	6	403219	5	NULL	NULL	0	NULL	electrodes 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphology and surface profiles of the electrodes examined by reflected light , electron , and atomic force microscopy were consistent with those of corrosion resistance , showing that the electrodes with higher corrosion resistance had lower surface roughness than others .
	manualset3
111933	7	403219	5	NULL	NULL	NULL	NULL	higher corrosion resistance	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Morphology and surface profiles of the electrodes examined by reflected light , electron , and atomic force microscopy were consistent with those of corrosion resistance , showing that the electrodes with higher corrosion resistance had lower surface roughness than others .
	manualset3
111934	8	403219	5	NULL	NULL	NULL	NULL	lower surface roughness	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Morphology and surface profiles of the electrodes examined by reflected light , electron , and atomic force microscopy were consistent with those of corrosion resistance , showing that the electrodes with higher corrosion resistance had lower surface roughness than others .
	manualset3
111935	1	403220	5	NULL	NULL	0	NULL	Morphometric analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphometric analysis of the capillary ultrastructure revealed that alterations in flow and appearance were associated with changes in the extension of pericyte processes .
	manualset3
111936	2	403220	5	NULL	NULL	0	NULL	capillary ultrastructure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphometric analysis of the capillary ultrastructure revealed that alterations in flow and appearance were associated with changes in the extension of pericyte processes .
	manualset3
111937	3	403220	5	NULL	NULL	0	NULL	alterations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphometric analysis of the capillary ultrastructure revealed that alterations in flow and appearance were associated with changes in the extension of pericyte processes .
	manualset3
111938	4	403220	5	NULL	NULL	0	NULL	flow 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphometric analysis of the capillary ultrastructure revealed that alterations in flow and appearance were associated with changes in the extension of pericyte processes .
	manualset3
111939	5	403220	5	NULL	NULL	0	NULL	appearance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphometric analysis of the capillary ultrastructure revealed that alterations in flow and appearance were associated with changes in the extension of pericyte processes .
	manualset3
111940	6	403220	5	NULL	NULL	0	NULL	changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphometric analysis of the capillary ultrastructure revealed that alterations in flow and appearance were associated with changes in the extension of pericyte processes .
	manualset3
111941	7	403220	5	NULL	NULL	0	NULL	extension 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphometric analysis of the capillary ultrastructure revealed that alterations in flow and appearance were associated with changes in the extension of pericyte processes .
	manualset3
111942	8	403220	5	NULL	NULL	NULL	NULL	pericyte processes	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Morphometric analysis of the capillary ultrastructure revealed that alterations in flow and appearance were associated with changes in the extension of pericyte processes .
	manualset3
111943	1	403221	5	NULL	NULL	0	NULL	Morphometric evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphometric evaluation by light microscopy indicated that the extent of decidualization in PGF2 alpha-treated tissue was comparable to that of scratch-treated tissue .
	manualset3
111944	2	403221	5	NULL	NULL	0	NULL	light microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphometric evaluation by light microscopy indicated that the extent of decidualization in PGF2 alpha-treated tissue was comparable to that of scratch-treated tissue .
	manualset3
111945	3	403221	5	NULL	NULL	0	NULL	extent 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphometric evaluation by light microscopy indicated that the extent of decidualization in PGF2 alpha-treated tissue was comparable to that of scratch-treated tissue .
	manualset3
111946	4	403221	5	NULL	NULL	0	NULL	decidualization 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphometric evaluation by light microscopy indicated that the extent of decidualization in PGF2 alpha-treated tissue was comparable to that of scratch-treated tissue .
	manualset3
111947	5	403221	5	NULL	NULL	0	NULL	PGF2 alpha-treated tissue 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphometric evaluation by light microscopy indicated that the extent of decidualization in PGF2 alpha-treated tissue was comparable to that of scratch-treated tissue .
	manualset3
111948	6	403221	5	NULL	NULL	0	NULL	scratch-treated tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphometric evaluation by light microscopy indicated that the extent of decidualization in PGF2 alpha-treated tissue was comparable to that of scratch-treated tissue .
	manualset3
111949	1	403222	5	NULL	NULL	0	NULL	Morphometric study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphometric study of the lens in staged human embryos .
	manualset3
111950	2	403222	5	NULL	NULL	0	NULL	lens 	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphometric study of the lens in staged human embryos .
	manualset3
111951	3	403222	5	NULL	NULL	0	NULL	staged human embryos	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphometric study of the lens in staged human embryos .
	manualset3
111952	1	403223	5	NULL	NULL	0	NULL	Mortality 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality ( & lt ; 30 days ) was 3.5 % following aorto-iliac bypass in the treatment of arterial occlusive disease and 8.4 % after aneurysm repair ( asymptomatic , symptomatic and ruptured aneurysms all included ) .
	manualset3
111953	2	403223	5	NULL	NULL	0	NULL	 lt ; 30 days	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality ( & lt ; 30 days ) was 3.5 % following aorto-iliac bypass in the treatment of arterial occlusive disease and 8.4 % after aneurysm repair ( asymptomatic , symptomatic and ruptured aneurysms all included ) .
	manualset3
111954	3	403223	5	NULL	NULL	0	NULL	3.5 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality ( & lt ; 30 days ) was 3.5 % following aorto-iliac bypass in the treatment of arterial occlusive disease and 8.4 % after aneurysm repair ( asymptomatic , symptomatic and ruptured aneurysms all included ) .
	manualset3
111955	4	403223	5	NULL	NULL	0	NULL	aorto-iliac bypass	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality ( & lt ; 30 days ) was 3.5 % following aorto-iliac bypass in the treatment of arterial occlusive disease and 8.4 % after aneurysm repair ( asymptomatic , symptomatic and ruptured aneurysms all included ) .
	manualset3
111956	5	403223	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality ( & lt ; 30 days ) was 3.5 % following aorto-iliac bypass in the treatment of arterial occlusive disease and 8.4 % after aneurysm repair ( asymptomatic , symptomatic and ruptured aneurysms all included ) .
	manualset3
111957	6	403223	5	NULL	NULL	0	NULL	arterial occlusive disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality ( & lt ; 30 days ) was 3.5 % following aorto-iliac bypass in the treatment of arterial occlusive disease and 8.4 % after aneurysm repair ( asymptomatic , symptomatic and ruptured aneurysms all included ) .
	manualset3
111958	7	403223	5	NULL	NULL	0	NULL	8.4 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality ( & lt ; 30 days ) was 3.5 % following aorto-iliac bypass in the treatment of arterial occlusive disease and 8.4 % after aneurysm repair ( asymptomatic , symptomatic and ruptured aneurysms all included ) .
	manualset3
111959	8	403223	5	NULL	NULL	0	NULL	aneurysm repair 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality ( & lt ; 30 days ) was 3.5 % following aorto-iliac bypass in the treatment of arterial occlusive disease and 8.4 % after aneurysm repair ( asymptomatic , symptomatic and ruptured aneurysms all included ) .
	manualset3
111960	9	403223	5	NULL	NULL	0	NULL	asymptomatic aneurysms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality ( & lt ; 30 days ) was 3.5 % following aorto-iliac bypass in the treatment of arterial occlusive disease and 8.4 % after aneurysm repair ( asymptomatic , symptomatic and ruptured aneurysms all included ) .
	manualset3
111961	10	403223	5	NULL	NULL	0	NULL	symptomatic aneurysms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality ( & lt ; 30 days ) was 3.5 % following aorto-iliac bypass in the treatment of arterial occlusive disease and 8.4 % after aneurysm repair ( asymptomatic , symptomatic and ruptured aneurysms all included ) .
	manualset3
111962	11	403223	5	NULL	NULL	0	NULL	ruptured aneurysms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality ( & lt ; 30 days ) was 3.5 % following aorto-iliac bypass in the treatment of arterial occlusive disease and 8.4 % after aneurysm repair ( asymptomatic , symptomatic and ruptured aneurysms all included ) .
	manualset3
111963	1	403224	5	NULL	NULL	0	NULL	chromosomal cluster of genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A chromosomal cluster of genes encoding ADP-glucose synthetase , glycogen synthase and phosphoglucomutase in Agrobacterium tumefaciens .
	manualset3
111964	2	403224	5	NULL	NULL	0	NULL	ADP-glucose synthetase	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A chromosomal cluster of genes encoding ADP-glucose synthetase , glycogen synthase and phosphoglucomutase in Agrobacterium tumefaciens .
	manualset3
111965	3	403224	5	NULL	NULL	0	NULL	glycogen synthase	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A chromosomal cluster of genes encoding ADP-glucose synthetase , glycogen synthase and phosphoglucomutase in Agrobacterium tumefaciens .
	manualset3
111966	4	403224	5	NULL	NULL	0	NULL	phosphoglucomutase 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A chromosomal cluster of genes encoding ADP-glucose synthetase , glycogen synthase and phosphoglucomutase in Agrobacterium tumefaciens .
	manualset3
111967	5	403224	5	NULL	NULL	0	NULL	Agrobacterium tumefaciens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A chromosomal cluster of genes encoding ADP-glucose synthetase , glycogen synthase and phosphoglucomutase in Agrobacterium tumefaciens .
	manualset3
111968	1	403225	5	NULL	NULL	NULL	NULL	Mortality 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mortality and morbidity are high , and early diagnosis and appropriate antimicrobial treatment are essential .
	manualset3
111969	2	403225	5	NULL	NULL	0	NULL	morbidity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality and morbidity are high , and early diagnosis and appropriate antimicrobial treatment are essential .
	manualset3
111970	3	403225	5	NULL	NULL	NULL	NULL	early diagnosis 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mortality and morbidity are high , and early diagnosis and appropriate antimicrobial treatment are essential .
	manualset3
111971	4	403225	5	NULL	NULL	NULL	NULL	appropriate antimicrobial treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mortality and morbidity are high , and early diagnosis and appropriate antimicrobial treatment are essential .
	manualset3
111972	1	403226	5	NULL	NULL	0	NULL	Mortality experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality experience of Navajos with type 2 diabetes mellitus .
	manualset3
111973	2	403226	5	NULL	NULL	0	NULL	Navajos 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality experience of Navajos with type 2 diabetes mellitus .
	manualset3
111974	3	403226	5	NULL	NULL	0	NULL	type 2 diabetes mellitus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality experience of Navajos with type 2 diabetes mellitus .
	manualset3
111975	1	403227	5	NULL	NULL	0	NULL	Mortality 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality from liver disease in the West Midlands , 1993-2000 : observational study .
	manualset3
111976	2	403227	5	NULL	NULL	0	NULL	liver disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality from liver disease in the West Midlands , 1993-2000 : observational study .
	manualset3
111977	3	403227	5	NULL	NULL	0	NULL	 West Midlands	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality from liver disease in the West Midlands , 1993-2000 : observational study .
	manualset3
111978	4	403227	5	NULL	NULL	0	NULL	1993-2000	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality from liver disease in the West Midlands , 1993-2000 : observational study .
	manualset3
111979	5	403227	5	NULL	NULL	0	NULL	observational study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality from liver disease in the West Midlands , 1993-2000 : observational study .
	manualset3
111980	1	403228	5	NULL	NULL	0	NULL	Mortality 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality from lung cancer among workers employed in formaldehyde industries .
	manualset3
111981	2	403228	5	NULL	NULL	0	NULL	lung cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality from lung cancer among workers employed in formaldehyde industries .
	manualset3
111982	3	403228	5	NULL	NULL	0	NULL	workers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality from lung cancer among workers employed in formaldehyde industries .
	manualset3
111983	4	403228	5	NULL	NULL	0	NULL	formaldehyde industries	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality from lung cancer among workers employed in formaldehyde industries .
	manualset3
111984	1	403229	5	NULL	NULL	0	NULL	Mortality 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality in patients with atrial fibrillation has significantly decreased during the last three decades : 35 years of follow-up in 1627 pacemaker patients .
	manualset3
111985	2	403229	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality in patients with atrial fibrillation has significantly decreased during the last three decades : 35 years of follow-up in 1627 pacemaker patients .
	manualset3
111986	3	403229	5	NULL	NULL	0	NULL	atrial fibrillation	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality in patients with atrial fibrillation has significantly decreased during the last three decades : 35 years of follow-up in 1627 pacemaker patients .
	manualset3
111987	4	403229	5	NULL	NULL	0	NULL	last three decades	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality in patients with atrial fibrillation has significantly decreased during the last three decades : 35 years of follow-up in 1627 pacemaker patients .
	manualset3
111988	5	403229	5	NULL	NULL	0	NULL	35 years	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality in patients with atrial fibrillation has significantly decreased during the last three decades : 35 years of follow-up in 1627 pacemaker patients .
	manualset3
111989	6	403229	5	NULL	NULL	0	NULL	follow-up 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality in patients with atrial fibrillation has significantly decreased during the last three decades : 35 years of follow-up in 1627 pacemaker patients .
	manualset3
111990	7	403229	5	NULL	NULL	0	NULL	1627 pacemaker patients	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality in patients with atrial fibrillation has significantly decreased during the last three decades : 35 years of follow-up in 1627 pacemaker patients .
	manualset3
111991	1	403230	5	NULL	NULL	0	NULL	Mortality 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality of iron-steel workers in Anshan , China : a retrospective cohort study .
	manualset3
111992	2	403230	5	NULL	NULL	0	NULL	iron-steel workers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality of iron-steel workers in Anshan , China : a retrospective cohort study .
	manualset3
111993	3	403230	5	NULL	NULL	0	NULL	Anshan , China	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality of iron-steel workers in Anshan , China : a retrospective cohort study .
	manualset3
111994	4	403230	5	NULL	NULL	0	NULL	retrospective cohort study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality of iron-steel workers in Anshan , China : a retrospective cohort study .
	manualset3
111995	1	403231	5	NULL	NULL	0	NULL	Mortality study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality study of workers in a polyvinyl-chloride production plant .
	manualset3
111996	2	403231	5	NULL	NULL	0	NULL	workers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality study of workers in a polyvinyl-chloride production plant .
	manualset3
111997	3	403231	5	NULL	NULL	0	NULL	polyvinyl-chloride production plant	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality study of workers in a polyvinyl-chloride production plant .
	manualset3
111998	1	403232	5	NULL	NULL	0	NULL	Morton 's neuroma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Morton 's neuroma : a review of recent concepts .
	manualset3
111999	2	403232	5	NULL	NULL	0	NULL	review 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Morton 's neuroma : a review of recent concepts .
	manualset3
112000	3	403232	5	NULL	NULL	0	NULL	recent concepts 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Morton 's neuroma : a review of recent concepts .
	manualset3
112001	1	403233	5	NULL	NULL	0	NULL	chronic inflammatory process	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A chronic inflammatory process with activation of microglial cells contribute to the neurodegeneration associated with Alzheimer 's disease ( AD ) .
	manualset3
112002	2	403233	5	NULL	NULL	0	NULL	activation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A chronic inflammatory process with activation of microglial cells contribute to the neurodegeneration associated with Alzheimer 's disease ( AD ) .
	manualset3
112003	3	403233	5	NULL	NULL	0	NULL	microglial cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A chronic inflammatory process with activation of microglial cells contribute to the neurodegeneration associated with Alzheimer 's disease ( AD ) .
	manualset3
112004	4	403233	5	NULL	NULL	0	NULL	neurodegeneration 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A chronic inflammatory process with activation of microglial cells contribute to the neurodegeneration associated with Alzheimer 's disease ( AD ) .
	manualset3
112005	5	403233	5	NULL	NULL	0	NULL	Alzheimer 's disease ( AD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A chronic inflammatory process with activation of microglial cells contribute to the neurodegeneration associated with Alzheimer 's disease ( AD ) .
	manualset3
112006	1	403234	5	NULL	NULL	0	NULL	Mosquito-induced infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mosquito-induced infection with equine encephalomyelitis virus in dogs .
	manualset3
112007	2	403234	5	NULL	NULL	0	NULL	equine encephalomyelitis virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mosquito-induced infection with equine encephalomyelitis virus in dogs .
	manualset3
112008	3	403234	5	NULL	NULL	0	NULL	dogs 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mosquito-induced infection with equine encephalomyelitis virus in dogs .
	manualset3
112009	1	403235	5	NULL	NULL	0	NULL	Mossy cell loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mossy cell loss and mossy fiber sprouting are two characteristic consequences of repeated seizures and head trauma .
	manualset3
112010	2	403235	5	NULL	NULL	0	NULL	mossy fiber sprouting	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mossy cell loss and mossy fiber sprouting are two characteristic consequences of repeated seizures and head trauma .
	manualset3
112011	3	403235	5	NULL	NULL	0	NULL	characteristic consequences 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mossy cell loss and mossy fiber sprouting are two characteristic consequences of repeated seizures and head trauma .
	manualset3
112012	4	403235	5	NULL	NULL	0	NULL	repeated seizures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mossy cell loss and mossy fiber sprouting are two characteristic consequences of repeated seizures and head trauma .
	manualset3
112013	5	403235	5	NULL	NULL	0	NULL	head trauma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mossy cell loss and mossy fiber sprouting are two characteristic consequences of repeated seizures and head trauma .
	manualset3
112014	1	403236	5	NULL	NULL	0	NULL	 99 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Most ( 99 % ) of the HP-N was of low molecular mass and consisted mainly of HP-N-30 .
	manualset3
112015	2	403236	5	NULL	NULL	0	NULL	HP-N	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Most ( 99 % ) of the HP-N was of low molecular mass and consisted mainly of HP-N-30 .
	manualset3
112016	3	403236	5	NULL	NULL	0	NULL	low molecular mass	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Most ( 99 % ) of the HP-N was of low molecular mass and consisted mainly of HP-N-30 .
	manualset3
112017	4	403236	5	NULL	NULL	0	NULL	HP-N-30	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Most ( 99 % ) of the HP-N was of low molecular mass and consisted mainly of HP-N-30 .
	manualset3
112018	1	403237	5	NULL	NULL	0	NULL	cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Most cases of superficial esophageal cancer have been reported in Japan and China .
	manualset3
112019	2	403237	5	NULL	NULL	0	NULL	superficial esophageal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Most cases of superficial esophageal cancer have been reported in Japan and China .
	manualset3
112020	3	403237	5	NULL	NULL	0	NULL	Japan 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Most cases of superficial esophageal cancer have been reported in Japan and China .
	manualset3
112021	4	403237	5	NULL	NULL	0	NULL	China 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Most cases of superficial esophageal cancer have been reported in Japan and China .
	manualset3
112022	1	403238	5	NULL	NULL	0	NULL	drug abuse treatment agencies	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Most drug abuse treatment agencies maintain a wide array of ancillary services , either on-site or through off-site referral resources , for helping meet the diverse social , medical , and psychological needs of clients .
	manualset3
112023	2	403238	5	NULL	NULL	0	NULL	wide array 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Most drug abuse treatment agencies maintain a wide array of ancillary services , either on-site or through off-site referral resources , for helping meet the diverse social , medical , and psychological needs of clients .
	manualset3
112024	3	403238	5	NULL	NULL	0	NULL	ancillary services 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most drug abuse treatment agencies maintain a wide array of ancillary services , either on-site or through off-site referral resources , for helping meet the diverse social , medical , and psychological needs of clients .
	manualset3
112025	4	403238	5	NULL	NULL	0	NULL	on-site referral resources	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Most drug abuse treatment agencies maintain a wide array of ancillary services , either on-site or through off-site referral resources , for helping meet the diverse social , medical , and psychological needs of clients .
	manualset3
112026	5	403238	5	NULL	NULL	0	NULL	off-site referral resources	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Most drug abuse treatment agencies maintain a wide array of ancillary services , either on-site or through off-site referral resources , for helping meet the diverse social , medical , and psychological needs of clients .
	manualset3
112027	6	403238	5	NULL	NULL	0	NULL	social needs	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most drug abuse treatment agencies maintain a wide array of ancillary services , either on-site or through off-site referral resources , for helping meet the diverse social , medical , and psychological needs of clients .
	manualset3
112028	7	403238	5	NULL	NULL	0	NULL	medical needs	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most drug abuse treatment agencies maintain a wide array of ancillary services , either on-site or through off-site referral resources , for helping meet the diverse social , medical , and psychological needs of clients .
	manualset3
112029	8	403238	5	NULL	NULL	0	NULL	psychological needs	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most drug abuse treatment agencies maintain a wide array of ancillary services , either on-site or through off-site referral resources , for helping meet the diverse social , medical , and psychological needs of clients .
	manualset3
112030	9	403238	5	NULL	NULL	0	NULL	clients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Most drug abuse treatment agencies maintain a wide array of ancillary services , either on-site or through off-site referral resources , for helping meet the diverse social , medical , and psychological needs of clients .
	manualset3
112031	1	403239	5	NULL	NULL	0	NULL	dynamin 2 mutants	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Most dynamin 2 mutants partially decreased clathrin-mediated endocytosis when ectopically expressed in cultured cells ; however , experiments in patient fibroblasts suggested that endocytosis is overall not defective .
	manualset3
112032	2	403239	5	NULL	NULL	0	NULL	clathrin-mediated endocytosis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Most dynamin 2 mutants partially decreased clathrin-mediated endocytosis when ectopically expressed in cultured cells ; however , experiments in patient fibroblasts suggested that endocytosis is overall not defective .
	manualset3
112033	3	403239	5	NULL	NULL	0	NULL	cultured cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Most dynamin 2 mutants partially decreased clathrin-mediated endocytosis when ectopically expressed in cultured cells ; however , experiments in patient fibroblasts suggested that endocytosis is overall not defective .
	manualset3
112034	4	403239	5	NULL	NULL	0	NULL	experiments 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Most dynamin 2 mutants partially decreased clathrin-mediated endocytosis when ectopically expressed in cultured cells ; however , experiments in patient fibroblasts suggested that endocytosis is overall not defective .
	manualset3
112035	5	403239	5	NULL	NULL	0	NULL	patient fibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Most dynamin 2 mutants partially decreased clathrin-mediated endocytosis when ectopically expressed in cultured cells ; however , experiments in patient fibroblasts suggested that endocytosis is overall not defective .
	manualset3
112036	6	403239	5	NULL	NULL	0	NULL	endocytosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Most dynamin 2 mutants partially decreased clathrin-mediated endocytosis when ectopically expressed in cultured cells ; however , experiments in patient fibroblasts suggested that endocytosis is overall not defective .
	manualset3
112037	1	403240	5	NULL	NULL	NULL	NULL	classification 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A classification of the subfamily Phlebotominae .
	manualset3
112038	2	403240	5	NULL	NULL	NULL	NULL	subfamily Phlebotominae	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A classification of the subfamily Phlebotominae .
	manualset3
112039	1	403241	5	NULL	NULL	0	NULL	experts 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Most experts agree , that there is the need for large clinical trials to determine the accuracy and precision of MDCT for triage of patients with acute chest pain .
	manualset3
112040	2	403241	5	NULL	NULL	0	NULL	clinical trials 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Most experts agree , that there is the need for large clinical trials to determine the accuracy and precision of MDCT for triage of patients with acute chest pain .
	manualset3
112041	3	403241	5	NULL	NULL	0	NULL	accuracy 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most experts agree , that there is the need for large clinical trials to determine the accuracy and precision of MDCT for triage of patients with acute chest pain .
	manualset3
112042	4	403241	5	NULL	NULL	0	NULL	precision 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most experts agree , that there is the need for large clinical trials to determine the accuracy and precision of MDCT for triage of patients with acute chest pain .
	manualset3
112043	5	403241	5	NULL	NULL	NULL	NULL	MDCT 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Most experts agree , that there is the need for large clinical trials to determine the accuracy and precision of MDCT for triage of patients with acute chest pain .
	manualset3
112044	6	403241	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Most experts agree , that there is the need for large clinical trials to determine the accuracy and precision of MDCT for triage of patients with acute chest pain .
	manualset3
112045	7	403241	5	NULL	NULL	0	NULL	acute chest pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Most experts agree , that there is the need for large clinical trials to determine the accuracy and precision of MDCT for triage of patients with acute chest pain .
	manualset3
112046	1	403242	5	NULL	NULL	0	NULL	genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Most genes of the VH4 family were used with various D-J combinations and a relatively high frequency of somatic mutations .
	manualset3
112047	2	403242	5	NULL	NULL	0	NULL	VH4 family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Most genes of the VH4 family were used with various D-J combinations and a relatively high frequency of somatic mutations .
	manualset3
112048	3	403242	5	NULL	NULL	0	NULL	D-J combinations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Most genes of the VH4 family were used with various D-J combinations and a relatively high frequency of somatic mutations .
	manualset3
112049	4	403242	5	NULL	NULL	0	NULL	high frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Most genes of the VH4 family were used with various D-J combinations and a relatively high frequency of somatic mutations .
	manualset3
112050	5	403242	5	NULL	NULL	0	NULL	somatic mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Most genes of the VH4 family were used with various D-J combinations and a relatively high frequency of somatic mutations .
	manualset3
112051	1	403243	5	NULL	NULL	0	NULL	hovering animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Most hovering animals , such as insects and hummingbirds , enhance lift by producing leading edge vortices ( LEVs ) and by using both the downstroke and upstroke for lift production .
	manualset3
112052	2	403243	5	NULL	NULL	0	NULL	insects 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Most hovering animals , such as insects and hummingbirds , enhance lift by producing leading edge vortices ( LEVs ) and by using both the downstroke and upstroke for lift production .
	manualset3
112053	3	403243	5	NULL	NULL	0	NULL	hummingbirds 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Most hovering animals , such as insects and hummingbirds , enhance lift by producing leading edge vortices ( LEVs ) and by using both the downstroke and upstroke for lift production .
	manualset3
112054	4	403243	5	NULL	NULL	0	NULL	lift 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most hovering animals , such as insects and hummingbirds , enhance lift by producing leading edge vortices ( LEVs ) and by using both the downstroke and upstroke for lift production .
	manualset3
112055	5	403243	5	NULL	NULL	0	NULL	leading edge vortices ( LEVs ) 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most hovering animals , such as insects and hummingbirds , enhance lift by producing leading edge vortices ( LEVs ) and by using both the downstroke and upstroke for lift production .
	manualset3
112056	6	403243	5	NULL	NULL	0	NULL	downstroke 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most hovering animals , such as insects and hummingbirds , enhance lift by producing leading edge vortices ( LEVs ) and by using both the downstroke and upstroke for lift production .
	manualset3
112057	7	403243	5	NULL	NULL	0	NULL	upstroke 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most hovering animals , such as insects and hummingbirds , enhance lift by producing leading edge vortices ( LEVs ) and by using both the downstroke and upstroke for lift production .
	manualset3
112058	8	403243	5	NULL	NULL	0	NULL	lift production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most hovering animals , such as insects and hummingbirds , enhance lift by producing leading edge vortices ( LEVs ) and by using both the downstroke and upstroke for lift production .
	manualset3
112059	1	403244	5	NULL	NULL	0	NULL	hypersensitivity reactions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Most hypersensitivity reactions to drugs occur within several weeks of administration ; signs and symptoms are often consistent with known immune-mediated reactions , including anaphylaxis , rashes , fever , cytopenias and vasculitis .
	manualset3
112060	2	403244	5	NULL	NULL	0	NULL	drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Most hypersensitivity reactions to drugs occur within several weeks of administration ; signs and symptoms are often consistent with known immune-mediated reactions , including anaphylaxis , rashes , fever , cytopenias and vasculitis .
	manualset3
112061	3	403244	5	NULL	NULL	0	NULL	several weeks	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Most hypersensitivity reactions to drugs occur within several weeks of administration ; signs and symptoms are often consistent with known immune-mediated reactions , including anaphylaxis , rashes , fever , cytopenias and vasculitis .
	manualset3
112062	4	403244	5	NULL	NULL	0	NULL	administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Most hypersensitivity reactions to drugs occur within several weeks of administration ; signs and symptoms are often consistent with known immune-mediated reactions , including anaphylaxis , rashes , fever , cytopenias and vasculitis .
	manualset3
112063	5	403244	5	NULL	NULL	0	NULL	signs 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Most hypersensitivity reactions to drugs occur within several weeks of administration ; signs and symptoms are often consistent with known immune-mediated reactions , including anaphylaxis , rashes , fever , cytopenias and vasculitis .
	manualset3
112064	6	403244	5	NULL	NULL	0	NULL	symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Most hypersensitivity reactions to drugs occur within several weeks of administration ; signs and symptoms are often consistent with known immune-mediated reactions , including anaphylaxis , rashes , fever , cytopenias and vasculitis .
	manualset3
112065	7	403244	5	NULL	NULL	0	NULL	immune-mediated reactions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Most hypersensitivity reactions to drugs occur within several weeks of administration ; signs and symptoms are often consistent with known immune-mediated reactions , including anaphylaxis , rashes , fever , cytopenias and vasculitis .
	manualset3
112066	8	403244	5	NULL	NULL	0	NULL	anaphylaxis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Most hypersensitivity reactions to drugs occur within several weeks of administration ; signs and symptoms are often consistent with known immune-mediated reactions , including anaphylaxis , rashes , fever , cytopenias and vasculitis .
	manualset3
112067	9	403244	5	NULL	NULL	0	NULL	rashes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Most hypersensitivity reactions to drugs occur within several weeks of administration ; signs and symptoms are often consistent with known immune-mediated reactions , including anaphylaxis , rashes , fever , cytopenias and vasculitis .
	manualset3
112068	10	403244	5	NULL	NULL	0	NULL	fever 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Most hypersensitivity reactions to drugs occur within several weeks of administration ; signs and symptoms are often consistent with known immune-mediated reactions , including anaphylaxis , rashes , fever , cytopenias and vasculitis .
	manualset3
112069	11	403244	5	NULL	NULL	0	NULL	cytopenias 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Most hypersensitivity reactions to drugs occur within several weeks of administration ; signs and symptoms are often consistent with known immune-mediated reactions , including anaphylaxis , rashes , fever , cytopenias and vasculitis .
	manualset3
112070	12	403244	5	NULL	NULL	0	NULL	vasculitis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Most hypersensitivity reactions to drugs occur within several weeks of administration ; signs and symptoms are often consistent with known immune-mediated reactions , including anaphylaxis , rashes , fever , cytopenias and vasculitis .
	manualset3
112071	1	403245	5	NULL	NULL	0	NULL	in vivo data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Most in vivo data are consistent with a model in which expansion and deletion occur by different mechanisms .
	manualset3
112072	2	403245	5	NULL	NULL	0	NULL	model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Most in vivo data are consistent with a model in which expansion and deletion occur by different mechanisms .
	manualset3
112073	3	403245	5	NULL	NULL	0	NULL	expansion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most in vivo data are consistent with a model in which expansion and deletion occur by different mechanisms .
	manualset3
112074	4	403245	5	NULL	NULL	0	NULL	deletion 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Most in vivo data are consistent with a model in which expansion and deletion occur by different mechanisms .
	manualset3
112075	5	403245	5	NULL	NULL	0	NULL	mechanisms 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most in vivo data are consistent with a model in which expansion and deletion occur by different mechanisms .
	manualset3
112076	1	403246	5	NULL	NULL	0	NULL	mosquitoes 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Most mosquitoes placed in a 1.0-gauss , uniform magnetic field moved until they were oriented parallel to the field .
	manualset3
112077	2	403246	5	NULL	NULL	0	NULL	1.0-gauss	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Most mosquitoes placed in a 1.0-gauss , uniform magnetic field moved until they were oriented parallel to the field .
	manualset3
112078	3	403246	5	NULL	NULL	0	NULL	uniform magnetic field	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Most mosquitoes placed in a 1.0-gauss , uniform magnetic field moved until they were oriented parallel to the field .
	manualset3
112079	4	403246	5	NULL	NULL	0	NULL	field 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Most mosquitoes placed in a 1.0-gauss , uniform magnetic field moved until they were oriented parallel to the field .
	manualset3
112080	1	403247	5	NULL	NULL	0	NULL	membrane-bound HNE	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of membrane-bound HNE and Pr3 can be released from the membrane surface of fixed cells by a buffer containing detergent , suggesting that hydrophobic interactions are involved in membrane binding .
	manualset3
112081	2	403247	5	NULL	NULL	0	NULL	Pr3 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of membrane-bound HNE and Pr3 can be released from the membrane surface of fixed cells by a buffer containing detergent , suggesting that hydrophobic interactions are involved in membrane binding .
	manualset3
112082	3	403247	5	NULL	NULL	0	NULL	membrane surface 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of membrane-bound HNE and Pr3 can be released from the membrane surface of fixed cells by a buffer containing detergent , suggesting that hydrophobic interactions are involved in membrane binding .
	manualset3
112083	4	403247	5	NULL	NULL	0	NULL	fixed cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of membrane-bound HNE and Pr3 can be released from the membrane surface of fixed cells by a buffer containing detergent , suggesting that hydrophobic interactions are involved in membrane binding .
	manualset3
112084	5	403247	5	NULL	NULL	0	NULL	buffer 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of membrane-bound HNE and Pr3 can be released from the membrane surface of fixed cells by a buffer containing detergent , suggesting that hydrophobic interactions are involved in membrane binding .
	manualset3
112085	6	403247	5	NULL	NULL	0	NULL	detergent 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of membrane-bound HNE and Pr3 can be released from the membrane surface of fixed cells by a buffer containing detergent , suggesting that hydrophobic interactions are involved in membrane binding .
	manualset3
112086	7	403247	5	NULL	NULL	0	NULL	hydrophobic interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of membrane-bound HNE and Pr3 can be released from the membrane surface of fixed cells by a buffer containing detergent , suggesting that hydrophobic interactions are involved in membrane binding .
	manualset3
112087	1	403248	5	NULL	NULL	NULL	NULL	 108 compounds 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Most of the 108 compounds recorded were of isoprenoid origin , but only 28 of the compounds were found in all 62 samples analyzed .
	manualset3
112088	2	403248	5	NULL	NULL	0	NULL	isoprenoid origin	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the 108 compounds recorded were of isoprenoid origin , but only 28 of the compounds were found in all 62 samples analyzed .
	manualset3
112089	3	403248	5	NULL	NULL	0	NULL	28	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the 108 compounds recorded were of isoprenoid origin , but only 28 of the compounds were found in all 62 samples analyzed .
	manualset3
112090	4	403248	5	NULL	NULL	0	NULL	compounds 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the 108 compounds recorded were of isoprenoid origin , but only 28 of the compounds were found in all 62 samples analyzed .
	manualset3
112091	5	403248	5	NULL	NULL	NULL	NULL	62 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Most of the 108 compounds recorded were of isoprenoid origin , but only 28 of the compounds were found in all 62 samples analyzed .
	manualset3
112981	6	403248	5	NULL	NULL	0	NULL	samples	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the 108 compounds recorded were of isoprenoid origin , but only 28 of the compounds were found in all 62 samples analyzed .
	manualset3
112113	1	403249	5	NULL	NULL	0	NULL	BOSCC sera	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the BOSCC sera reacted with autologous and allogeneic BOSCC cells and did not show any significant reactivity with normal skin cells ( autologous or allogeneic ) .
	manualset3
112116	2	403249	5	NULL	NULL	0	NULL	autologous BOSCC cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the BOSCC sera reacted with autologous and allogeneic BOSCC cells and did not show any significant reactivity with normal skin cells ( autologous or allogeneic ) .
	manualset3
112118	3	403249	5	NULL	NULL	0	NULL	allogeneic BOSCC cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the BOSCC sera reacted with autologous and allogeneic BOSCC cells and did not show any significant reactivity with normal skin cells ( autologous or allogeneic ) .
	manualset3
112120	4	403249	5	NULL	NULL	0	NULL	reactivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the BOSCC sera reacted with autologous and allogeneic BOSCC cells and did not show any significant reactivity with normal skin cells ( autologous or allogeneic ) .
	manualset3
112122	5	403249	5	NULL	NULL	0	NULL	normal skin cells ( autologous or allogeneic )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the BOSCC sera reacted with autologous and allogeneic BOSCC cells and did not show any significant reactivity with normal skin cells ( autologous or allogeneic ) .
	manualset3
112123	1	403250	5	NULL	NULL	0	NULL	definition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A clear definition of target areas to be investigated is a prerequisite for successful future efforts in this area .
	manualset3
112124	2	403250	5	NULL	NULL	0	NULL	target areas	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A clear definition of target areas to be investigated is a prerequisite for successful future efforts in this area .
	manualset3
112125	3	403250	5	NULL	NULL	0	NULL	prerequisite	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A clear definition of target areas to be investigated is a prerequisite for successful future efforts in this area .
	manualset3
112126	4	403250	5	NULL	NULL	0	NULL	successful future efforts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A clear definition of target areas to be investigated is a prerequisite for successful future efforts in this area .
	manualset3
112127	5	403250	5	NULL	NULL	0	NULL	area	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A clear definition of target areas to be investigated is a prerequisite for successful future efforts in this area .
	manualset3
112128	1	403251	5	NULL	NULL	0	NULL	Mn reduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the Mn reduction in these sediments may have been coupled to the oxidation of acid volatile sulfides ( AVS ) , rather than to dissimilatory reduction .
	manualset3
112129	2	403251	5	NULL	NULL	0	NULL	sediments	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the Mn reduction in these sediments may have been coupled to the oxidation of acid volatile sulfides ( AVS ) , rather than to dissimilatory reduction .
	manualset3
112130	3	403251	5	NULL	NULL	0	NULL	oxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the Mn reduction in these sediments may have been coupled to the oxidation of acid volatile sulfides ( AVS ) , rather than to dissimilatory reduction .
	manualset3
112131	4	403251	5	NULL	NULL	0	NULL	acid volatile sulfides ( AVS ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the Mn reduction in these sediments may have been coupled to the oxidation of acid volatile sulfides ( AVS ) , rather than to dissimilatory reduction .
	manualset3
112132	5	403251	5	NULL	NULL	0	NULL	dissimilatory reduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the Mn reduction in these sediments may have been coupled to the oxidation of acid volatile sulfides ( AVS ) , rather than to dissimilatory reduction .
	manualset3
112133	1	403252	5	NULL	NULL	0	NULL	airborne cobalt	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the airborne cobalt was water soluble ( ionized ) , but there was also solid particles containing cobalt and other materials in the air of the workplaces .
	manualset3
112134	2	403252	5	NULL	NULL	0	NULL	solid particles containing cobalt	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the airborne cobalt was water soluble ( ionized ) , but there was also solid particles containing cobalt and other materials in the air of the workplaces .
	manualset3
112135	3	403252	5	NULL	NULL	0	NULL	materials	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the airborne cobalt was water soluble ( ionized ) , but there was also solid particles containing cobalt and other materials in the air of the workplaces .
	manualset3
112136	4	403252	5	NULL	NULL	0	NULL	air	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the airborne cobalt was water soluble ( ionized ) , but there was also solid particles containing cobalt and other materials in the air of the workplaces .
	manualset3
112137	5	403252	5	NULL	NULL	0	NULL	workplaces	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the airborne cobalt was water soluble ( ionized ) , but there was also solid particles containing cobalt and other materials in the air of the workplaces .
	manualset3
112138	1	403253	5	NULL	NULL	0	NULL	binding sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the binding sites were found to be occupied by endogenous estrogen ( s ) .
	manualset3
112139	2	403253	5	NULL	NULL	0	NULL	endogenous estrogen ( s )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the binding sites were found to be occupied by endogenous estrogen ( s ) .
	manualset3
112140	1	403254	5	NULL	NULL	0	NULL	discussions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the discussions focused on interest rates , the education system , and the culture -- all very interesting but not very useful .
	manualset3
112141	2	403254	5	NULL	NULL	0	NULL	interest rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the discussions focused on interest rates , the education system , and the culture -- all very interesting but not very useful .
	manualset3
112202	3	403254	5	NULL	NULL	0	NULL	education system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the discussions focused on interest rates , the education system , and the culture -- all very interesting but not very useful .
	manualset3
112203	4	403254	5	NULL	NULL	0	NULL	culture 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the discussions focused on interest rates , the education system , and the culture -- all very interesting but not very useful .
	manualset3
112204	1	403255	5	NULL	NULL	0	NULL	hydrocarbon substrates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the hydrocarbon and carboxylic acid substrates resulted in a mixture of sophorolipids consisting of free acids and the more desirable lactones .
	manualset3
112205	2	403255	5	NULL	NULL	0	NULL	carboxylic acid substrates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the hydrocarbon and carboxylic acid substrates resulted in a mixture of sophorolipids consisting of free acids and the more desirable lactones .
	manualset3
112206	3	403255	5	NULL	NULL	0	NULL	mixture 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the hydrocarbon and carboxylic acid substrates resulted in a mixture of sophorolipids consisting of free acids and the more desirable lactones .
	manualset3
112207	4	403255	5	NULL	NULL	0	NULL	sophorolipids 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the hydrocarbon and carboxylic acid substrates resulted in a mixture of sophorolipids consisting of free acids and the more desirable lactones .
	manualset3
112208	5	403255	5	NULL	NULL	0	NULL	free acids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the hydrocarbon and carboxylic acid substrates resulted in a mixture of sophorolipids consisting of free acids and the more desirable lactones .
	manualset3
112209	6	403255	5	NULL	NULL	NULL	NULL	lactones 	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Most of the hydrocarbon and carboxylic acid substrates resulted in a mixture of sophorolipids consisting of free acids and the more desirable lactones .
	manualset3
112210	1	403256	5	NULL	NULL	0	NULL	observed cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the observed cells showed a standing gradient of calcium , the calcium concentrations in the distal dendritic end of the cell being higher than in the soma .
	manualset3
112211	2	403256	5	NULL	NULL	0	NULL	standing gradient	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the observed cells showed a standing gradient of calcium , the calcium concentrations in the distal dendritic end of the cell being higher than in the soma .
	manualset3
112212	3	403256	5	NULL	NULL	0	NULL	calcium 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the observed cells showed a standing gradient of calcium , the calcium concentrations in the distal dendritic end of the cell being higher than in the soma .
	manualset3
112213	4	403256	5	NULL	NULL	0	NULL	calcium concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the observed cells showed a standing gradient of calcium , the calcium concentrations in the distal dendritic end of the cell being higher than in the soma .
	manualset3
112214	5	403256	5	NULL	NULL	0	NULL	distal dendritic end	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the observed cells showed a standing gradient of calcium , the calcium concentrations in the distal dendritic end of the cell being higher than in the soma .
	manualset3
112215	6	403256	5	NULL	NULL	0	NULL	cell 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the observed cells showed a standing gradient of calcium , the calcium concentrations in the distal dendritic end of the cell being higher than in the soma .
	manualset3
112216	7	403256	5	NULL	NULL	0	NULL	soma 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the observed cells showed a standing gradient of calcium , the calcium concentrations in the distal dendritic end of the cell being higher than in the soma .
	manualset3
112217	1	403257	5	NULL	NULL	0	NULL	 previous works 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the previous works focused on the phase transition of the water droplet phase .
	manualset3
112218	2	403257	5	NULL	NULL	0	NULL	phase transition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the previous works focused on the phase transition of the water droplet phase .
	manualset3
112219	3	403257	5	NULL	NULL	0	NULL	water droplet phase	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the previous works focused on the phase transition of the water droplet phase .
	manualset3
112220	1	403258	5	NULL	NULL	0	NULL	radioactivity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the radioactivity in plasma up to 8 hr after dosing was due to the parent drug .
	manualset3
112221	2	403258	5	NULL	NULL	NULL	NULL	plasma 	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Most of the radioactivity in plasma up to 8 hr after dosing was due to the parent drug .
	manualset3
112222	3	403258	5	NULL	NULL	0	NULL	8 hr 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the radioactivity in plasma up to 8 hr after dosing was due to the parent drug .
	manualset3
112223	4	403258	5	NULL	NULL	0	NULL	parent drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the radioactivity in plasma up to 8 hr after dosing was due to the parent drug .
	manualset3
112224	1	403259	5	NULL	NULL	NULL	NULL	samples 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Most of the samples fall in C3S1 quality with high salinity hazard and low sodium hazard .
	manualset3
112225	2	403259	5	NULL	NULL	0	NULL	C3S1 quality	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the samples fall in C3S1 quality with high salinity hazard and low sodium hazard .
	manualset3
112226	3	403259	5	NULL	NULL	0	NULL	high salinity hazard	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the samples fall in C3S1 quality with high salinity hazard and low sodium hazard .
	manualset3
112227	4	403259	5	NULL	NULL	0	NULL	low sodium hazard	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the samples fall in C3S1 quality with high salinity hazard and low sodium hazard .
	manualset3
112228	1	403260	5	NULL	NULL	NULL	NULL	sorbents 	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Most of the sorbents employed in this study ( homogeneous lithocomponents separated from aquifer sediments or fresh rock fragments ) showed highly nonlinear sorption isotherms because of coal particles embedded inside the grains .
	manualset3
112229	2	403260	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the sorbents employed in this study ( homogeneous lithocomponents separated from aquifer sediments or fresh rock fragments ) showed highly nonlinear sorption isotherms because of coal particles embedded inside the grains .
	manualset3
112230	3	403260	5	NULL	NULL	NULL	NULL	homogeneous lithocomponents	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Most of the sorbents employed in this study ( homogeneous lithocomponents separated from aquifer sediments or fresh rock fragments ) showed highly nonlinear sorption isotherms because of coal particles embedded inside the grains .
	manualset3
112231	4	403260	5	NULL	NULL	NULL	NULL	aquifer sediments	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Most of the sorbents employed in this study ( homogeneous lithocomponents separated from aquifer sediments or fresh rock fragments ) showed highly nonlinear sorption isotherms because of coal particles embedded inside the grains .
	manualset3
112232	5	403260	5	NULL	NULL	NULL	NULL	fresh rock fragments	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Most of the sorbents employed in this study ( homogeneous lithocomponents separated from aquifer sediments or fresh rock fragments ) showed highly nonlinear sorption isotherms because of coal particles embedded inside the grains .
	manualset3
112233	6	403260	5	NULL	NULL	0	NULL	highly nonlinear sorption isotherms	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the sorbents employed in this study ( homogeneous lithocomponents separated from aquifer sediments or fresh rock fragments ) showed highly nonlinear sorption isotherms because of coal particles embedded inside the grains .
	manualset3
112234	7	403260	5	NULL	NULL	0	NULL	coal particles	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the sorbents employed in this study ( homogeneous lithocomponents separated from aquifer sediments or fresh rock fragments ) showed highly nonlinear sorption isotherms because of coal particles embedded inside the grains .
	manualset3
112235	8	403260	5	NULL	NULL	0	NULL	grains 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the sorbents employed in this study ( homogeneous lithocomponents separated from aquifer sediments or fresh rock fragments ) showed highly nonlinear sorption isotherms because of coal particles embedded inside the grains .
	manualset3
112236	1	403261	5	NULL	NULL	0	NULL	species 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the species of Euphorbiaceae are known to be toxic and poisonous plants because their milky latex has strong skin irritant activity , and chronic exposure can result carcinogenic effect .
	manualset3
112237	2	403261	5	NULL	NULL	0	NULL	Euphorbiaceae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the species of Euphorbiaceae are known to be toxic and poisonous plants because their milky latex has strong skin irritant activity , and chronic exposure can result carcinogenic effect .
	manualset3
112238	3	403261	5	NULL	NULL	0	NULL	toxic plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the species of Euphorbiaceae are known to be toxic and poisonous plants because their milky latex has strong skin irritant activity , and chronic exposure can result carcinogenic effect .
	manualset3
112239	4	403261	5	NULL	NULL	0	NULL	poisonous plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the species of Euphorbiaceae are known to be toxic and poisonous plants because their milky latex has strong skin irritant activity , and chronic exposure can result carcinogenic effect .
	manualset3
112240	5	403261	5	NULL	NULL	0	NULL	milky latex	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the species of Euphorbiaceae are known to be toxic and poisonous plants because their milky latex has strong skin irritant activity , and chronic exposure can result carcinogenic effect .
	manualset3
112241	6	403261	5	NULL	NULL	0	NULL	strong skin irritant activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the species of Euphorbiaceae are known to be toxic and poisonous plants because their milky latex has strong skin irritant activity , and chronic exposure can result carcinogenic effect .
	manualset3
112242	7	403261	5	NULL	NULL	0	NULL	chronic exposure 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the species of Euphorbiaceae are known to be toxic and poisonous plants because their milky latex has strong skin irritant activity , and chronic exposure can result carcinogenic effect .
	manualset3
112243	8	403261	5	NULL	NULL	0	NULL	carcinogenic effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the species of Euphorbiaceae are known to be toxic and poisonous plants because their milky latex has strong skin irritant activity , and chronic exposure can result carcinogenic effect .
	manualset3
112244	1	403262	5	NULL	NULL	0	NULL	Biguanide-induced lactic acidosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Biguanide-induced and - associated lactic acidosis : serum and tissue biguanide levels in hyperlactemia and lactic acidosis ( author 's transl ) ) .
	manualset3
112245	2	403262	5	NULL	NULL	0	NULL	Biguanide- associated lactic acidosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Biguanide-induced and - associated lactic acidosis : serum and tissue biguanide levels in hyperlactemia and lactic acidosis ( author 's transl ) ) .
	manualset3
112246	3	403262	5	NULL	NULL	0	NULL	serum biguanide levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Biguanide-induced and - associated lactic acidosis : serum and tissue biguanide levels in hyperlactemia and lactic acidosis ( author 's transl ) ) .
	manualset3
112247	4	403262	5	NULL	NULL	0	NULL	tissue biguanide levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Biguanide-induced and - associated lactic acidosis : serum and tissue biguanide levels in hyperlactemia and lactic acidosis ( author 's transl ) ) .
	manualset3
112248	5	403262	5	NULL	NULL	NULL	NULL	hyperlactemia 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Biguanide-induced and - associated lactic acidosis : serum and tissue biguanide levels in hyperlactemia and lactic acidosis ( author 's transl ) ) .
	manualset3
112249	6	403262	5	NULL	NULL	0	NULL	lactic acidosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Biguanide-induced and - associated lactic acidosis : serum and tissue biguanide levels in hyperlactemia and lactic acidosis ( author 's transl ) ) .
	manualset3
112250	1	403263	5	NULL	NULL	0	NULL	editing sites	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of these editing sites are confined to intramolecular hairpin double-stranded RNA ( dsRNA ) structures formed by pairing of neighboring , reversely oriented , primate-specific Alu repeats .
	manualset3
112251	2	403263	5	NULL	NULL	0	NULL	intramolecular hairpin double-stranded RNA ( dsRNA ) structures	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of these editing sites are confined to intramolecular hairpin double-stranded RNA ( dsRNA ) structures formed by pairing of neighboring , reversely oriented , primate-specific Alu repeats .
	manualset3
112252	3	403263	5	NULL	NULL	0	NULL	reversely oriented , primate-specific Alu repeats	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of these editing sites are confined to intramolecular hairpin double-stranded RNA ( dsRNA ) structures formed by pairing of neighboring , reversely oriented , primate-specific Alu repeats .
	manualset3
112253	1	403264	5	NULL	NULL	0	NULL	accurate location	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of these involve the accurate location of masses and , as in angiography , projections in several planes are essential .
	manualset3
112254	2	403264	5	NULL	NULL	0	NULL	masses 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of these involve the accurate location of masses and , as in angiography , projections in several planes are essential .
	manualset3
112255	3	403264	5	NULL	NULL	0	NULL	angiography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of these involve the accurate location of masses and , as in angiography , projections in several planes are essential .
	manualset3
112256	4	403264	5	NULL	NULL	0	NULL	projections 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of these involve the accurate location of masses and , as in angiography , projections in several planes are essential .
	manualset3
112257	5	403264	5	NULL	NULL	0	NULL	several planes 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of these involve the accurate location of masses and , as in angiography , projections in several planes are essential .
	manualset3
112258	1	403265	5	NULL	NULL	0	NULL	mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of these mutations are paternal in origin , but the male : female mutation rate ratio is currently uncertain and might vary even among individuals within a population .
	manualset3
112259	2	403265	5	NULL	NULL	0	NULL	origin 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of these mutations are paternal in origin , but the male : female mutation rate ratio is currently uncertain and might vary even among individuals within a population .
	manualset3
112260	3	403265	5	NULL	NULL	0	NULL	male : female mutation rate ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of these mutations are paternal in origin , but the male : female mutation rate ratio is currently uncertain and might vary even among individuals within a population .
	manualset3
112261	4	403265	5	NULL	NULL	0	NULL	individuals 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of these mutations are paternal in origin , but the male : female mutation rate ratio is currently uncertain and might vary even among individuals within a population .
	manualset3
112262	5	403265	5	NULL	NULL	0	NULL	population 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of these mutations are paternal in origin , but the male : female mutation rate ratio is currently uncertain and might vary even among individuals within a population .
	manualset3
112263	1	403266	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Most patients lacked FOXP3-expressing cells , further solidifying the association between FOXP3 deficiency and immune dysregulation , polyendocrinopathy , enteropathy , X-linked syndrome .
	manualset3
112264	2	403266	5	NULL	NULL	0	NULL	FOXP3-expressing cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Most patients lacked FOXP3-expressing cells , further solidifying the association between FOXP3 deficiency and immune dysregulation , polyendocrinopathy , enteropathy , X-linked syndrome .
	manualset3
112265	3	403266	5	NULL	NULL	0	NULL	association 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Most patients lacked FOXP3-expressing cells , further solidifying the association between FOXP3 deficiency and immune dysregulation , polyendocrinopathy , enteropathy , X-linked syndrome .
	manualset3
112266	4	403266	5	NULL	NULL	0	NULL	FOXP3 deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Most patients lacked FOXP3-expressing cells , further solidifying the association between FOXP3 deficiency and immune dysregulation , polyendocrinopathy , enteropathy , X-linked syndrome .
	manualset3
112267	5	403266	5	NULL	NULL	NULL	NULL	immune dysregulation , polyendocrinopathy , enteropathy , X-linked syndrome	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Most patients lacked FOXP3-expressing cells , further solidifying the association between FOXP3 deficiency and immune dysregulation , polyendocrinopathy , enteropathy , X-linked syndrome .
	manualset3
112271	1	403267	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Most patients may therefore choose the most convenient time of day to inhale dornase alfa provided that they wait at least 30 minutes before performing ACT .
	manualset3
112272	2	403267	5	NULL	NULL	0	NULL	convenient time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Most patients may therefore choose the most convenient time of day to inhale dornase alfa provided that they wait at least 30 minutes before performing ACT .
	manualset3
112273	3	403267	5	NULL	NULL	0	NULL	day 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Most patients may therefore choose the most convenient time of day to inhale dornase alfa provided that they wait at least 30 minutes before performing ACT .
	manualset3
112274	4	403267	5	NULL	NULL	0	NULL	dornase alfa	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Most patients may therefore choose the most convenient time of day to inhale dornase alfa provided that they wait at least 30 minutes before performing ACT .
	manualset3
112275	5	403267	5	NULL	NULL	0	NULL	 30 minutes	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Most patients may therefore choose the most convenient time of day to inhale dornase alfa provided that they wait at least 30 minutes before performing ACT .
	manualset3
112276	6	403267	5	NULL	NULL	0	NULL	ACT 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Most patients may therefore choose the most convenient time of day to inhale dornase alfa provided that they wait at least 30 minutes before performing ACT .
	manualset3
112277	1	403268	5	NULL	NULL	0	NULL	plant microRNAs ( miRNAs )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Most plant microRNAs ( miRNAs ) have perfect or near-perfect complementarity with their targets .
	manualset3
112278	2	403268	5	NULL	NULL	0	NULL	complementarity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most plant microRNAs ( miRNAs ) have perfect or near-perfect complementarity with their targets .
	manualset3
112279	3	403268	5	NULL	NULL	0	NULL	targets	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Most plant microRNAs ( miRNAs ) have perfect or near-perfect complementarity with their targets .
	manualset3
112280	1	403269	5	NULL	NULL	0	NULL	research 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Most research and current clinical practice uses flashing lights and/or animated toys to provide reinforcement to a child during VRA .
	manualset3
112281	2	403269	5	NULL	NULL	0	NULL	current clinical practice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Most research and current clinical practice uses flashing lights and/or animated toys to provide reinforcement to a child during VRA .
	manualset3
112282	3	403269	5	NULL	NULL	0	NULL	flashing lights 	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Most research and current clinical practice uses flashing lights and/or animated toys to provide reinforcement to a child during VRA .
	manualset3
112283	4	403269	5	NULL	NULL	0	NULL	animated toys 	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Most research and current clinical practice uses flashing lights and/or animated toys to provide reinforcement to a child during VRA .
	manualset3
112284	5	403269	5	NULL	NULL	0	NULL	reinforcement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most research and current clinical practice uses flashing lights and/or animated toys to provide reinforcement to a child during VRA .
	manualset3
112285	6	403269	5	NULL	NULL	NULL	NULL	child 	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Most research and current clinical practice uses flashing lights and/or animated toys to provide reinforcement to a child during VRA .
	manualset3
112286	7	403269	5	NULL	NULL	0	NULL	VRA 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Most research and current clinical practice uses flashing lights and/or animated toys to provide reinforcement to a child during VRA .
	manualset3
112287	1	403270	5	NULL	NULL	0	NULL	clinical comparison 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A clinical and pharmacological comparison of chlorpropamide and other sulfonylureas .
	manualset3
112288	2	403270	5	NULL	NULL	0	NULL	pharmacological comparison	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A clinical and pharmacological comparison of chlorpropamide and other sulfonylureas .
	manualset3
112289	3	403270	5	NULL	NULL	0	NULL	chlorpropamide 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A clinical and pharmacological comparison of chlorpropamide and other sulfonylureas .
	manualset3
112290	4	403270	5	NULL	NULL	0	NULL	sulfonylureas 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A clinical and pharmacological comparison of chlorpropamide and other sulfonylureas .
	manualset3
112291	1	403271	5	NULL	NULL	0	NULL	species 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Most species were increased 2-3-fold , but some ( C16 : 0 / C20 : 4 and C18 : 0 / C20 : 4 ) were increased 3-6-fold .
	manualset3
112292	2	403271	5	NULL	NULL	0	NULL	2-3-fold	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Most species were increased 2-3-fold , but some ( C16 : 0 / C20 : 4 and C18 : 0 / C20 : 4 ) were increased 3-6-fold .
	manualset3
112293	3	403271	5	NULL	NULL	0	NULL	C16 : 0 / C20 : 4 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Most species were increased 2-3-fold , but some ( C16 : 0 / C20 : 4 and C18 : 0 / C20 : 4 ) were increased 3-6-fold .
	manualset3
112294	4	403271	5	NULL	NULL	0	NULL	C18 : 0 / C20 : 4	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Most species were increased 2-3-fold , but some ( C16 : 0 / C20 : 4 and C18 : 0 / C20 : 4 ) were increased 3-6-fold .
	manualset3
112295	5	403271	5	NULL	NULL	0	NULL	3-6-fold	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Most species were increased 2-3-fold , but some ( C16 : 0 / C20 : 4 and C18 : 0 / C20 : 4 ) were increased 3-6-fold .
	manualset3
112296	1	403272	5	NULL	NULL	NULL	NULL	samples 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Most these samples were also active for heterotypic gag-protein of HIV-1 serotype , p55 and p24 .
	manualset3
112297	2	403272	5	NULL	NULL	0	NULL	heterotypic gag-protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Most these samples were also active for heterotypic gag-protein of HIV-1 serotype , p55 and p24 .
	manualset3
112298	3	403272	5	NULL	NULL	0	NULL	HIV-1 serotype 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Most these samples were also active for heterotypic gag-protein of HIV-1 serotype , p55 and p24 .
	manualset3
112299	4	403272	5	NULL	NULL	0	NULL	p55 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Most these samples were also active for heterotypic gag-protein of HIV-1 serotype , p55 and p24 .
	manualset3
112300	5	403272	5	NULL	NULL	0	NULL	p24 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Most these samples were also active for heterotypic gag-protein of HIV-1 serotype , p55 and p24 .
	manualset3
112301	1	403273	5	NULL	NULL	0	NULL	variation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most variation in weight was explained by testing age , although treatment affected weight gain for the lead-6 gulls , particularly after 20 days .
	manualset3
112302	2	403273	5	NULL	NULL	0	NULL	weight 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Most variation in weight was explained by testing age , although treatment affected weight gain for the lead-6 gulls , particularly after 20 days .
	manualset3
112303	3	403273	5	NULL	NULL	0	NULL	age 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Most variation in weight was explained by testing age , although treatment affected weight gain for the lead-6 gulls , particularly after 20 days .
	manualset3
112304	4	403273	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Most variation in weight was explained by testing age , although treatment affected weight gain for the lead-6 gulls , particularly after 20 days .
	manualset3
112305	5	403273	5	NULL	NULL	0	NULL	weight gain	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most variation in weight was explained by testing age , although treatment affected weight gain for the lead-6 gulls , particularly after 20 days .
	manualset3
112306	6	403273	5	NULL	NULL	0	NULL	lead-6 gulls 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Most variation in weight was explained by testing age , although treatment affected weight gain for the lead-6 gulls , particularly after 20 days .
	manualset3
112307	7	403273	5	NULL	NULL	0	NULL	 after 20 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Most variation in weight was explained by testing age , although treatment affected weight gain for the lead-6 gulls , particularly after 20 days .
	manualset3
112308	1	403274	5	NULL	NULL	0	NULL	women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Most women who had worked in the garment industry for more than a year had changed factories at least once and been promoted from helper to operator , with attendant income increases .
	manualset3
112309	2	403274	5	NULL	NULL	0	NULL	garment industry 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Most women who had worked in the garment industry for more than a year had changed factories at least once and been promoted from helper to operator , with attendant income increases .
	manualset3
112310	3	403274	5	NULL	NULL	0	NULL	year 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Most women who had worked in the garment industry for more than a year had changed factories at least once and been promoted from helper to operator , with attendant income increases .
	manualset3
112311	4	403274	5	NULL	NULL	0	NULL	factories 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Most women who had worked in the garment industry for more than a year had changed factories at least once and been promoted from helper to operator , with attendant income increases .
	manualset3
112312	5	403274	5	NULL	NULL	0	NULL	helper 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Most women who had worked in the garment industry for more than a year had changed factories at least once and been promoted from helper to operator , with attendant income increases .
	manualset3
112313	6	403274	5	NULL	NULL	0	NULL	operator 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Most women who had worked in the garment industry for more than a year had changed factories at least once and been promoted from helper to operator , with attendant income increases .
	manualset3
112314	7	403274	5	NULL	NULL	0	NULL	attendant income	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Most women who had worked in the garment industry for more than a year had changed factories at least once and been promoted from helper to operator , with attendant income increases .
	manualset3
112315	1	403275	5	NULL	NULL	0	NULL	experimental models 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Most experimental models of allograft tolerance depend on manipulation of immune responses at the time of transplant .
	manualset3
112316	2	403275	5	NULL	NULL	0	NULL	allograft tolerance 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Most experimental models of allograft tolerance depend on manipulation of immune responses at the time of transplant .
	manualset3
112317	3	403275	5	NULL	NULL	0	NULL	manipulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most experimental models of allograft tolerance depend on manipulation of immune responses at the time of transplant .
	manualset3
112318	4	403275	5	NULL	NULL	0	NULL	immune responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Most experimental models of allograft tolerance depend on manipulation of immune responses at the time of transplant .
	manualset3
112319	5	403275	5	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Most experimental models of allograft tolerance depend on manipulation of immune responses at the time of transplant .
	manualset3
112320	6	403275	5	NULL	NULL	0	NULL	transplant 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Most experimental models of allograft tolerance depend on manipulation of immune responses at the time of transplant .
	manualset3
112321	1	403276	5	NULL	NULL	0	NULL	renal abnormalities 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Most renal abnormalities emerge within the first few years of SLE diagnosis .
	manualset3
112322	2	403276	5	NULL	NULL	0	NULL	first few years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Most renal abnormalities emerge within the first few years of SLE diagnosis .
	manualset3
112323	3	403276	5	NULL	NULL	NULL	NULL	SLE diagnosis 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Most renal abnormalities emerge within the first few years of SLE diagnosis .
	manualset3
112324	1	403277	5	NULL	NULL	0	NULL	PGC column	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Most important , the PGC column had a useful lifetime of five months and 500 sample analyses/column .
	manualset3
112325	2	403277	5	NULL	NULL	0	NULL	lifetime 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Most important , the PGC column had a useful lifetime of five months and 500 sample analyses/column .
	manualset3
112326	3	403277	5	NULL	NULL	0	NULL	five months	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Most important , the PGC column had a useful lifetime of five months and 500 sample analyses/column .
	manualset3
112327	4	403277	5	NULL	NULL	0	NULL	500 sample analyses/column	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Most important , the PGC column had a useful lifetime of five months and 500 sample analyses/column .
	manualset3
112328	1	403278	5	NULL	NULL	0	NULL	clinically stable residual subluxation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A clinically stable residual subluxation was present in 5 patients .
	manualset3
112329	2	403278	5	NULL	NULL	NULL	NULL	5 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A clinically stable residual subluxation was present in 5 patients .
	manualset3
112330	1	403279	5	NULL	NULL	0	NULL	2-fold increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Most obvious was an up to approximately 2-fold increase in galactose content in wood from transgenic plants due to increased compression wood formation .
	manualset3
112331	2	403279	5	NULL	NULL	0	NULL	galactose content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Most obvious was an up to approximately 2-fold increase in galactose content in wood from transgenic plants due to increased compression wood formation .
	manualset3
112332	3	403279	5	NULL	NULL	0	NULL	wood 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	Most obvious was an up to approximately 2-fold increase in galactose content in wood from transgenic plants due to increased compression wood formation .
	manualset3
112333	4	403279	5	NULL	NULL	0	NULL	transgenic plants 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Most obvious was an up to approximately 2-fold increase in galactose content in wood from transgenic plants due to increased compression wood formation .
	manualset3
112334	5	403279	5	NULL	NULL	0	NULL	compression wood formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Most obvious was an up to approximately 2-fold increase in galactose content in wood from transgenic plants due to increased compression wood formation .
	manualset3
112335	1	403280	5	NULL	NULL	0	NULL	 long-term consequences 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Most common long-term consequences of bladder augmentation including chronic infections , bladder stones , perforation , and malignancy are described .
	manualset3
112336	2	403280	5	NULL	NULL	0	NULL	bladder augmentation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Most common long-term consequences of bladder augmentation including chronic infections , bladder stones , perforation , and malignancy are described .
	manualset3
112337	3	403280	5	NULL	NULL	0	NULL	chronic infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Most common long-term consequences of bladder augmentation including chronic infections , bladder stones , perforation , and malignancy are described .
	manualset3
112338	4	403280	5	NULL	NULL	0	NULL	bladder stones 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Most common long-term consequences of bladder augmentation including chronic infections , bladder stones , perforation , and malignancy are described .
	manualset3
112339	5	403280	5	NULL	NULL	0	NULL	perforation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Most common long-term consequences of bladder augmentation including chronic infections , bladder stones , perforation , and malignancy are described .
	manualset3
112340	6	403280	5	NULL	NULL	0	NULL	malignancy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Most common long-term consequences of bladder augmentation including chronic infections , bladder stones , perforation , and malignancy are described .
	manualset3
112341	1	403281	5	NULL	NULL	0	NULL	postoperative complication 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Most common postoperative complication was hypocalcemia with 5 % rate ( persistent in 0.7 % ) , then recurrent laryngeal nerve injury in 4.4 % patients or 2.9 % according to number of exposed nerves .
	manualset3
112342	2	403281	5	NULL	NULL	0	NULL	hypocalcemia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Most common postoperative complication was hypocalcemia with 5 % rate ( persistent in 0.7 % ) , then recurrent laryngeal nerve injury in 4.4 % patients or 2.9 % according to number of exposed nerves .
	manualset3
112343	3	403281	5	NULL	NULL	0	NULL	 5 % rate	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Most common postoperative complication was hypocalcemia with 5 % rate ( persistent in 0.7 % ) , then recurrent laryngeal nerve injury in 4.4 % patients or 2.9 % according to number of exposed nerves .
	manualset3
112344	4	403281	5	NULL	NULL	0	NULL	0.7 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Most common postoperative complication was hypocalcemia with 5 % rate ( persistent in 0.7 % ) , then recurrent laryngeal nerve injury in 4.4 % patients or 2.9 % according to number of exposed nerves .
	manualset3
112345	5	403281	5	NULL	NULL	0	NULL	recurrent laryngeal nerve injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Most common postoperative complication was hypocalcemia with 5 % rate ( persistent in 0.7 % ) , then recurrent laryngeal nerve injury in 4.4 % patients or 2.9 % according to number of exposed nerves .
	manualset3
112346	6	403281	5	NULL	NULL	0	NULL	4.4 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Most common postoperative complication was hypocalcemia with 5 % rate ( persistent in 0.7 % ) , then recurrent laryngeal nerve injury in 4.4 % patients or 2.9 % according to number of exposed nerves .
	manualset3
112347	7	403281	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Most common postoperative complication was hypocalcemia with 5 % rate ( persistent in 0.7 % ) , then recurrent laryngeal nerve injury in 4.4 % patients or 2.9 % according to number of exposed nerves .
	manualset3
112348	8	403281	5	NULL	NULL	0	NULL	2.9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Most common postoperative complication was hypocalcemia with 5 % rate ( persistent in 0.7 % ) , then recurrent laryngeal nerve injury in 4.4 % patients or 2.9 % according to number of exposed nerves .
	manualset3
112349	9	403281	5	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Most common postoperative complication was hypocalcemia with 5 % rate ( persistent in 0.7 % ) , then recurrent laryngeal nerve injury in 4.4 % patients or 2.9 % according to number of exposed nerves .
	manualset3
112350	10	403281	5	NULL	NULL	0	NULL	exposed nerves	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Most common postoperative complication was hypocalcemia with 5 % rate ( persistent in 0.7 % ) , then recurrent laryngeal nerve injury in 4.4 % patients or 2.9 % according to number of exposed nerves .
	manualset3
112351	1	403282	5	NULL	NULL	0	NULL	cytotoxic chemotherapy protocols	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Most cytotoxic chemotherapy protocols used in small animals are designed to have a low risk of adverse effects ; however , adverse events can occasionally occur .
	manualset3
112352	2	403282	5	NULL	NULL	0	NULL	small animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Most cytotoxic chemotherapy protocols used in small animals are designed to have a low risk of adverse effects ; however , adverse events can occasionally occur .
	manualset3
112353	3	403282	5	NULL	NULL	0	NULL	low risk	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most cytotoxic chemotherapy protocols used in small animals are designed to have a low risk of adverse effects ; however , adverse events can occasionally occur .
	manualset3
112354	4	403282	5	NULL	NULL	0	NULL	adverse effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Most cytotoxic chemotherapy protocols used in small animals are designed to have a low risk of adverse effects ; however , adverse events can occasionally occur .
	manualset3
112355	5	403282	5	NULL	NULL	0	NULL	adverse events 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most cytotoxic chemotherapy protocols used in small animals are designed to have a low risk of adverse effects ; however , adverse events can occasionally occur .
	manualset3
112356	1	403283	5	NULL	NULL	0	NULL	mammalian cell surfaces	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Most mammalian cell surfaces display two major sialic acids ( Sias ) , N-acetylneuraminic acid ( Neu5Ac ) and N-glycolylneuraminic acid ( Neu5Gc ) .
	manualset3
112357	2	403283	5	NULL	NULL	0	NULL	sialic acids ( Sias ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Most mammalian cell surfaces display two major sialic acids ( Sias ) , N-acetylneuraminic acid ( Neu5Ac ) and N-glycolylneuraminic acid ( Neu5Gc ) .
	manualset3
112358	3	403283	5	NULL	NULL	0	NULL	N-acetylneuraminic acid ( Neu5Ac )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Most mammalian cell surfaces display two major sialic acids ( Sias ) , N-acetylneuraminic acid ( Neu5Ac ) and N-glycolylneuraminic acid ( Neu5Gc ) .
	manualset3
112359	4	403283	5	NULL	NULL	0	NULL	N-glycolylneuraminic acid ( Neu5Gc )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Most mammalian cell surfaces display two major sialic acids ( Sias ) , N-acetylneuraminic acid ( Neu5Ac ) and N-glycolylneuraminic acid ( Neu5Gc ) .
	manualset3
112360	1	403284	5	NULL	NULL	0	NULL	synaptic inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Most synaptic inhibition in the brain arises from transmembrane fluxes of chloride ions ( Cl ( - ) ) , so imaging intracellular Cl ( - ) concentration ( ( Cl ( - ) ) ( i ) ) is , in principle , a natural way to visualize the spatiotemporal dynamics of inhibition .
	manualset3
112361	2	403284	5	NULL	NULL	0	NULL	brain 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Most synaptic inhibition in the brain arises from transmembrane fluxes of chloride ions ( Cl ( - ) ) , so imaging intracellular Cl ( - ) concentration ( ( Cl ( - ) ) ( i ) ) is , in principle , a natural way to visualize the spatiotemporal dynamics of inhibition .
	manualset3
112362	3	403284	5	NULL	NULL	NULL	NULL	transmembrane fluxes 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Most synaptic inhibition in the brain arises from transmembrane fluxes of chloride ions ( Cl ( - ) ) , so imaging intracellular Cl ( - ) concentration ( ( Cl ( - ) ) ( i ) ) is , in principle , a natural way to visualize the spatiotemporal dynamics of inhibition .
	manualset3
112363	4	403284	5	NULL	NULL	0	NULL	chloride ions ( Cl ( - ) ) 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Most synaptic inhibition in the brain arises from transmembrane fluxes of chloride ions ( Cl ( - ) ) , so imaging intracellular Cl ( - ) concentration ( ( Cl ( - ) ) ( i ) ) is , in principle , a natural way to visualize the spatiotemporal dynamics of inhibition .
	manualset3
112364	5	403284	5	NULL	NULL	0	NULL	intracellular Cl ( - ) concentration ( ( Cl ( - ) ) ( i ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Most synaptic inhibition in the brain arises from transmembrane fluxes of chloride ions ( Cl ( - ) ) , so imaging intracellular Cl ( - ) concentration ( ( Cl ( - ) ) ( i ) ) is , in principle , a natural way to visualize the spatiotemporal dynamics of inhibition .
	manualset3
112365	6	403284	5	NULL	NULL	0	NULL	principle 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most synaptic inhibition in the brain arises from transmembrane fluxes of chloride ions ( Cl ( - ) ) , so imaging intracellular Cl ( - ) concentration ( ( Cl ( - ) ) ( i ) ) is , in principle , a natural way to visualize the spatiotemporal dynamics of inhibition .
	manualset3
112366	7	403284	5	NULL	NULL	0	NULL	spatiotemporal dynamics	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Most synaptic inhibition in the brain arises from transmembrane fluxes of chloride ions ( Cl ( - ) ) , so imaging intracellular Cl ( - ) concentration ( ( Cl ( - ) ) ( i ) ) is , in principle , a natural way to visualize the spatiotemporal dynamics of inhibition .
	manualset3
112367	8	403284	5	NULL	NULL	0	NULL	inhibition 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Most synaptic inhibition in the brain arises from transmembrane fluxes of chloride ions ( Cl ( - ) ) , so imaging intracellular Cl ( - ) concentration ( ( Cl ( - ) ) ( i ) ) is , in principle , a natural way to visualize the spatiotemporal dynamics of inhibition .
	manualset3
112368	1	403285	5	NULL	NULL	0	NULL	individual efficacy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most do not support individual efficacy toward recovery , the ability to control use , or social use after treatment .
	manualset3
112369	2	403285	5	NULL	NULL	0	NULL	recovery 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most do not support individual efficacy toward recovery , the ability to control use , or social use after treatment .
	manualset3
112370	3	403285	5	NULL	NULL	0	NULL	ability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most do not support individual efficacy toward recovery , the ability to control use , or social use after treatment .
	manualset3
112373	4	403285	5	NULL	NULL	NULL	NULL	treatment 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Most do not support individual efficacy toward recovery , the ability to control use , or social use after treatment .
	manualset3
122144	5	403285	5	NULL	NULL	0	NULL	use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most do not support individual efficacy toward recovery , the ability to control use , or social use after treatment .
	manualset3
122145	6	403285	5	NULL	NULL	0	NULL	social use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most do not support individual efficacy toward recovery , the ability to control use , or social use after treatment .
	manualset3
112374	1	403286	5	NULL	NULL	0	NULL	tumor perfusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Most commonly , tumor perfusion is measured using rapid gradient T2-weighted imaging during bolus injection of gadolinium dimeglumine gadopentetate .
	manualset3
112375	2	403286	5	NULL	NULL	0	NULL	rapid gradient T2-weighted imaging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Most commonly , tumor perfusion is measured using rapid gradient T2-weighted imaging during bolus injection of gadolinium dimeglumine gadopentetate .
	manualset3
112376	3	403286	5	NULL	NULL	0	NULL	bolus injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Most commonly , tumor perfusion is measured using rapid gradient T2-weighted imaging during bolus injection of gadolinium dimeglumine gadopentetate .
	manualset3
112377	4	403286	5	NULL	NULL	0	NULL	gadolinium dimeglumine gadopentetate 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Most commonly , tumor perfusion is measured using rapid gradient T2-weighted imaging during bolus injection of gadolinium dimeglumine gadopentetate .
	manualset3
112378	1	403287	5	NULL	NULL	0	NULL	epitopes 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Most developmentally regulated epitopes identified on embryonal carcinoma cells and murine preimplantation embryos are associated with a glycoprotein-bound large glycan called embryoglycan .
	manualset3
112379	2	403287	5	NULL	NULL	0	NULL	embryonal carcinoma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Most developmentally regulated epitopes identified on embryonal carcinoma cells and murine preimplantation embryos are associated with a glycoprotein-bound large glycan called embryoglycan .
	manualset3
112380	3	403287	5	NULL	NULL	0	NULL	murine preimplantation embryos	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Most developmentally regulated epitopes identified on embryonal carcinoma cells and murine preimplantation embryos are associated with a glycoprotein-bound large glycan called embryoglycan .
	manualset3
112381	4	403287	5	NULL	NULL	0	NULL	glycoprotein-bound large glycan	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Most developmentally regulated epitopes identified on embryonal carcinoma cells and murine preimplantation embryos are associated with a glycoprotein-bound large glycan called embryoglycan .
	manualset3
112382	5	403287	5	NULL	NULL	0	NULL	embryoglycan 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Most developmentally regulated epitopes identified on embryonal carcinoma cells and murine preimplantation embryos are associated with a glycoprotein-bound large glycan called embryoglycan .
	manualset3
112383	1	403288	5	NULL	NULL	0	NULL	hypoxia responsiveness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most importantly , its hypoxia responsiveness is the most ample of all three genes , being strongly induced in the lungs , liver , kidney , brain , heart and testis .
	manualset3
112384	2	403288	5	NULL	NULL	0	NULL	three genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Most importantly , its hypoxia responsiveness is the most ample of all three genes , being strongly induced in the lungs , liver , kidney , brain , heart and testis .
	manualset3
112385	3	403288	5	NULL	NULL	0	NULL	lungs 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Most importantly , its hypoxia responsiveness is the most ample of all three genes , being strongly induced in the lungs , liver , kidney , brain , heart and testis .
	manualset3
112386	4	403288	5	NULL	NULL	0	NULL	liver 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Most importantly , its hypoxia responsiveness is the most ample of all three genes , being strongly induced in the lungs , liver , kidney , brain , heart and testis .
	manualset3
112387	5	403288	5	NULL	NULL	0	NULL	kidney 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Most importantly , its hypoxia responsiveness is the most ample of all three genes , being strongly induced in the lungs , liver , kidney , brain , heart and testis .
	manualset3
112388	6	403288	5	NULL	NULL	0	NULL	brain 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Most importantly , its hypoxia responsiveness is the most ample of all three genes , being strongly induced in the lungs , liver , kidney , brain , heart and testis .
	manualset3
112389	7	403288	5	NULL	NULL	0	NULL	heart 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Most importantly , its hypoxia responsiveness is the most ample of all three genes , being strongly induced in the lungs , liver , kidney , brain , heart and testis .
	manualset3
112390	8	403288	5	NULL	NULL	0	NULL	testis 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Most importantly , its hypoxia responsiveness is the most ample of all three genes , being strongly induced in the lungs , liver , kidney , brain , heart and testis .
	manualset3
112391	1	403289	5	NULL	NULL	0	NULL	clinicopathologic study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A clinicopathologic study on the peripheral nervous system of the aged .
	manualset3
112392	2	403289	5	NULL	NULL	0	NULL	peripheral nervous system	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A clinicopathologic study on the peripheral nervous system of the aged .
	manualset3
112393	3	403289	5	NULL	NULL	0	NULL	aged 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A clinicopathologic study on the peripheral nervous system of the aged .
	manualset3
112394	1	403290	5	NULL	NULL	NULL	NULL	antiviral activities	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Most interestingly , the notable selective antiviral and antiproliferative activities were achieved respectively for 2f and 3f by modulating the ribose sugar moiety into deprotected and protected forms while retaining a similar trifluoromethylphenylethynyltriazole as the nucleobase .
	manualset3
112395	2	403290	5	NULL	NULL	NULL	NULL	antiproliferative activities 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Most interestingly , the notable selective antiviral and antiproliferative activities were achieved respectively for 2f and 3f by modulating the ribose sugar moiety into deprotected and protected forms while retaining a similar trifluoromethylphenylethynyltriazole as the nucleobase .
	manualset3
112396	3	403290	5	NULL	NULL	0	NULL	2f	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Most interestingly , the notable selective antiviral and antiproliferative activities were achieved respectively for 2f and 3f by modulating the ribose sugar moiety into deprotected and protected forms while retaining a similar trifluoromethylphenylethynyltriazole as the nucleobase .
	manualset3
112397	4	403290	5	NULL	NULL	0	NULL	3f 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Most interestingly , the notable selective antiviral and antiproliferative activities were achieved respectively for 2f and 3f by modulating the ribose sugar moiety into deprotected and protected forms while retaining a similar trifluoromethylphenylethynyltriazole as the nucleobase .
	manualset3
112398	5	403290	5	NULL	NULL	0	NULL	ribose sugar moiety 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Most interestingly , the notable selective antiviral and antiproliferative activities were achieved respectively for 2f and 3f by modulating the ribose sugar moiety into deprotected and protected forms while retaining a similar trifluoromethylphenylethynyltriazole as the nucleobase .
	manualset3
112399	6	403290	5	NULL	NULL	0	NULL	deprotected form	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Most interestingly , the notable selective antiviral and antiproliferative activities were achieved respectively for 2f and 3f by modulating the ribose sugar moiety into deprotected and protected forms while retaining a similar trifluoromethylphenylethynyltriazole as the nucleobase .
	manualset3
112400	7	403290	5	NULL	NULL	0	NULL	protected forms	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Most interestingly , the notable selective antiviral and antiproliferative activities were achieved respectively for 2f and 3f by modulating the ribose sugar moiety into deprotected and protected forms while retaining a similar trifluoromethylphenylethynyltriazole as the nucleobase .
	manualset3
112401	8	403290	5	NULL	NULL	0	NULL	trifluoromethylphenylethynyltriazole 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Most interestingly , the notable selective antiviral and antiproliferative activities were achieved respectively for 2f and 3f by modulating the ribose sugar moiety into deprotected and protected forms while retaining a similar trifluoromethylphenylethynyltriazole as the nucleobase .
	manualset3
112402	9	403290	5	NULL	NULL	0	NULL	nucleobase 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Most interestingly , the notable selective antiviral and antiproliferative activities were achieved respectively for 2f and 3f by modulating the ribose sugar moiety into deprotected and protected forms while retaining a similar trifluoromethylphenylethynyltriazole as the nucleobase .
	manualset3
112403	1	403291	5	NULL	NULL	0	NULL	tyrosine phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Most obviously , they suggest that tyrosine phosphorylation of a novel type of tyrosine kinase p125FAK is a point of convergence in the action of integrins , oncogenic forms of pp60src , mitogenic neuropeptides and growth factors ( Fig .
	manualset3
112404	2	403291	5	NULL	NULL	NULL	NULL	novel type	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Most obviously , they suggest that tyrosine phosphorylation of a novel type of tyrosine kinase p125FAK is a point of convergence in the action of integrins , oncogenic forms of pp60src , mitogenic neuropeptides and growth factors ( Fig .
	manualset3
112405	3	403291	5	NULL	NULL	0	NULL	tyrosine kinase p125FAK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Most obviously , they suggest that tyrosine phosphorylation of a novel type of tyrosine kinase p125FAK is a point of convergence in the action of integrins , oncogenic forms of pp60src , mitogenic neuropeptides and growth factors ( Fig .
	manualset3
112406	4	403291	5	NULL	NULL	0	NULL	convergence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most obviously , they suggest that tyrosine phosphorylation of a novel type of tyrosine kinase p125FAK is a point of convergence in the action of integrins , oncogenic forms of pp60src , mitogenic neuropeptides and growth factors ( Fig .
	manualset3
112407	5	403291	5	NULL	NULL	0	NULL	action 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most obviously , they suggest that tyrosine phosphorylation of a novel type of tyrosine kinase p125FAK is a point of convergence in the action of integrins , oncogenic forms of pp60src , mitogenic neuropeptides and growth factors ( Fig .
	manualset3
112408	6	403291	5	NULL	NULL	0	NULL	integrins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Most obviously , they suggest that tyrosine phosphorylation of a novel type of tyrosine kinase p125FAK is a point of convergence in the action of integrins , oncogenic forms of pp60src , mitogenic neuropeptides and growth factors ( Fig .
	manualset3
112409	7	403291	5	NULL	NULL	0	NULL	oncogenic forms of pp60src	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Most obviously , they suggest that tyrosine phosphorylation of a novel type of tyrosine kinase p125FAK is a point of convergence in the action of integrins , oncogenic forms of pp60src , mitogenic neuropeptides and growth factors ( Fig .
	manualset3
112410	8	403291	5	NULL	NULL	0	NULL	mitogenic neuropeptides 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Most obviously , they suggest that tyrosine phosphorylation of a novel type of tyrosine kinase p125FAK is a point of convergence in the action of integrins , oncogenic forms of pp60src , mitogenic neuropeptides and growth factors ( Fig .
	manualset3
112411	9	403291	5	NULL	NULL	0	NULL	growth factors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Most obviously , they suggest that tyrosine phosphorylation of a novel type of tyrosine kinase p125FAK is a point of convergence in the action of integrins , oncogenic forms of pp60src , mitogenic neuropeptides and growth factors ( Fig .
	manualset3
112412	1	403292	5	NULL	NULL	0	NULL	assay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Most recently , we have used this assay to examine lectin binding ligands on two human cell types , CCL-220 , a colon cancer cell line , and CRL-1459 , a non-cancer colon cell line .
	manualset3
112413	2	403292	5	NULL	NULL	0	NULL	lectin binding ligands	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Most recently , we have used this assay to examine lectin binding ligands on two human cell types , CCL-220 , a colon cancer cell line , and CRL-1459 , a non-cancer colon cell line .
	manualset3
112414	3	403292	5	NULL	NULL	0	NULL	 two human cell types	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Most recently , we have used this assay to examine lectin binding ligands on two human cell types , CCL-220 , a colon cancer cell line , and CRL-1459 , a non-cancer colon cell line .
	manualset3
112415	4	403292	5	NULL	NULL	0	NULL	CCL-220 , a colon cancer cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Most recently , we have used this assay to examine lectin binding ligands on two human cell types , CCL-220 , a colon cancer cell line , and CRL-1459 , a non-cancer colon cell line .
	manualset3
112416	5	403292	5	NULL	NULL	0	NULL	CRL-1459 , a non-cancer colon cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Most recently , we have used this assay to examine lectin binding ligands on two human cell types , CCL-220 , a colon cancer cell line , and CRL-1459 , a non-cancer colon cell line .
	manualset3
112417	1	403293	5	NULL	NULL	0	NULL	change 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most significantly there is a large change ( approximately 16 kcal/mol ) in the MOZYME MM component due to polarization of the MM region surrounding the active site , and which arises mostly from MM atoms close to ( & lt ; 10 A ) the active-site QM region , which is not modelled explicitly by our QM/MM method .
	manualset3
112418	2	403293	5	NULL	NULL	0	NULL	16 kcal/mol 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Most significantly there is a large change ( approximately 16 kcal/mol ) in the MOZYME MM component due to polarization of the MM region surrounding the active site , and which arises mostly from MM atoms close to ( & lt ; 10 A ) the active-site QM region , which is not modelled explicitly by our QM/MM method .
	manualset3
112419	3	403293	5	NULL	NULL	0	NULL	MOZYME MM component 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Most significantly there is a large change ( approximately 16 kcal/mol ) in the MOZYME MM component due to polarization of the MM region surrounding the active site , and which arises mostly from MM atoms close to ( & lt ; 10 A ) the active-site QM region , which is not modelled explicitly by our QM/MM method .
	manualset3
112420	4	403293	5	NULL	NULL	0	NULL	polarization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most significantly there is a large change ( approximately 16 kcal/mol ) in the MOZYME MM component due to polarization of the MM region surrounding the active site , and which arises mostly from MM atoms close to ( & lt ; 10 A ) the active-site QM region , which is not modelled explicitly by our QM/MM method .
	manualset3
112421	5	403293	5	NULL	NULL	NULL	NULL	MM region	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Most significantly there is a large change ( approximately 16 kcal/mol ) in the MOZYME MM component due to polarization of the MM region surrounding the active site , and which arises mostly from MM atoms close to ( & lt ; 10 A ) the active-site QM region , which is not modelled explicitly by our QM/MM method .
	manualset3
112422	6	403293	5	NULL	NULL	0	NULL	active site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Most significantly there is a large change ( approximately 16 kcal/mol ) in the MOZYME MM component due to polarization of the MM region surrounding the active site , and which arises mostly from MM atoms close to ( & lt ; 10 A ) the active-site QM region , which is not modelled explicitly by our QM/MM method .
	manualset3
112423	7	403293	5	NULL	NULL	0	NULL	MM atoms	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Most significantly there is a large change ( approximately 16 kcal/mol ) in the MOZYME MM component due to polarization of the MM region surrounding the active site , and which arises mostly from MM atoms close to ( & lt ; 10 A ) the active-site QM region , which is not modelled explicitly by our QM/MM method .
	manualset3
112424	8	403293	5	NULL	NULL	0	NULL	 lt ; 10 A	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Most significantly there is a large change ( approximately 16 kcal/mol ) in the MOZYME MM component due to polarization of the MM region surrounding the active site , and which arises mostly from MM atoms close to ( & lt ; 10 A ) the active-site QM region , which is not modelled explicitly by our QM/MM method .
	manualset3
112425	9	403293	5	NULL	NULL	0	NULL	active-site QM region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Most significantly there is a large change ( approximately 16 kcal/mol ) in the MOZYME MM component due to polarization of the MM region surrounding the active site , and which arises mostly from MM atoms close to ( & lt ; 10 A ) the active-site QM region , which is not modelled explicitly by our QM/MM method .
	manualset3
112426	10	403293	5	NULL	NULL	0	NULL	QM/MM method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Most significantly there is a large change ( approximately 16 kcal/mol ) in the MOZYME MM component due to polarization of the MM region surrounding the active site , and which arises mostly from MM atoms close to ( & lt ; 10 A ) the active-site QM region , which is not modelled explicitly by our QM/MM method .
	manualset3
112427	1	403294	5	NULL	NULL	0	NULL	Motion artifacts 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Motion artifacts arise from several sources , which include respiration , flow of fluids , and swallowing .
	manualset3
112428	2	403294	5	NULL	NULL	0	NULL	sources 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Motion artifacts arise from several sources , which include respiration , flow of fluids , and swallowing .
	manualset3
112429	3	403294	5	NULL	NULL	0	NULL	respiration 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Motion artifacts arise from several sources , which include respiration , flow of fluids , and swallowing .
	manualset3
112430	4	403294	5	NULL	NULL	0	NULL	flow of fluids	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Motion artifacts arise from several sources , which include respiration , flow of fluids , and swallowing .
	manualset3
112431	5	403294	5	NULL	NULL	0	NULL	swallowing 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Motion artifacts arise from several sources , which include respiration , flow of fluids , and swallowing .
	manualset3
112432	1	403295	5	NULL	NULL	0	NULL	success 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Motivated by the broad success of this approach , mission planners are now conceiving and demanding higher performance from space systems .
	manualset3
112433	2	403295	5	NULL	NULL	0	NULL	approach 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Motivated by the broad success of this approach , mission planners are now conceiving and demanding higher performance from space systems .
	manualset3
112434	3	403295	5	NULL	NULL	0	NULL	mission planners	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Motivated by the broad success of this approach , mission planners are now conceiving and demanding higher performance from space systems .
	manualset3
112435	4	403295	5	NULL	NULL	0	NULL	higher performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Motivated by the broad success of this approach , mission planners are now conceiving and demanding higher performance from space systems .
	manualset3
112436	5	403295	5	NULL	NULL	0	NULL	space systems	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Motivated by the broad success of this approach , mission planners are now conceiving and demanding higher performance from space systems .
	manualset3
112437	1	403296	5	NULL	NULL	0	NULL	Motor cortex organization 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Motor cortex organization after stroke is related to side of stroke and level of recovery .
	manualset3
112438	2	403296	5	NULL	NULL	0	NULL	stroke 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Motor cortex organization after stroke is related to side of stroke and level of recovery .
	manualset3
112439	3	403296	5	NULL	NULL	0	NULL	side 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Motor cortex organization after stroke is related to side of stroke and level of recovery .
	manualset3
112440	4	403296	5	NULL	NULL	0	NULL	stroke 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Motor cortex organization after stroke is related to side of stroke and level of recovery .
	manualset3
112441	5	403296	5	NULL	NULL	0	NULL	level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Motor cortex organization after stroke is related to side of stroke and level of recovery .
	manualset3
112442	6	403296	5	NULL	NULL	0	NULL	recovery 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Motor cortex organization after stroke is related to side of stroke and level of recovery .
	manualset3
112443	1	403297	5	NULL	NULL	0	NULL	Motor cortex stimulation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Motor cortex stimulation in a three-year-old child with trigeminal neuropathic pain caused by a malignant glioma in the cerebellopontine angle : case report .
	manualset3
112444	2	403297	5	NULL	NULL	0	NULL	three-year-old child	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Motor cortex stimulation in a three-year-old child with trigeminal neuropathic pain caused by a malignant glioma in the cerebellopontine angle : case report .
	manualset3
112445	3	403297	5	NULL	NULL	0	NULL	trigeminal neuropathic pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Motor cortex stimulation in a three-year-old child with trigeminal neuropathic pain caused by a malignant glioma in the cerebellopontine angle : case report .
	manualset3
112446	4	403297	5	NULL	NULL	0	NULL	malignant glioma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Motor cortex stimulation in a three-year-old child with trigeminal neuropathic pain caused by a malignant glioma in the cerebellopontine angle : case report .
	manualset3
112447	5	403297	5	NULL	NULL	0	NULL	cerebellopontine angle	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Motor cortex stimulation in a three-year-old child with trigeminal neuropathic pain caused by a malignant glioma in the cerebellopontine angle : case report .
	manualset3
112448	6	403297	5	NULL	NULL	0	NULL	case report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Motor cortex stimulation in a three-year-old child with trigeminal neuropathic pain caused by a malignant glioma in the cerebellopontine angle : case report .
	manualset3
112449	1	403298	5	NULL	NULL	0	NULL	Motor learning	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Motor learning and movement automatization were characterized by a significant reduction of theta ERS in the anterior cingulate cortex ( ACC ) , a ROI linked to focused attention , and with a shift of neuronal activation in alpha 2 band from the bilateral superior parietal areas to the homologous area of the left hemisphere .
	manualset3
112450	2	403298	5	NULL	NULL	0	NULL	movement automatization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Motor learning and movement automatization were characterized by a significant reduction of theta ERS in the anterior cingulate cortex ( ACC ) , a ROI linked to focused attention , and with a shift of neuronal activation in alpha 2 band from the bilateral superior parietal areas to the homologous area of the left hemisphere .
	manualset3
112451	3	403298	5	NULL	NULL	0	NULL	significant reduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Motor learning and movement automatization were characterized by a significant reduction of theta ERS in the anterior cingulate cortex ( ACC ) , a ROI linked to focused attention , and with a shift of neuronal activation in alpha 2 band from the bilateral superior parietal areas to the homologous area of the left hemisphere .
	manualset3
112452	4	403298	5	NULL	NULL	0	NULL	theta ERS 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Motor learning and movement automatization were characterized by a significant reduction of theta ERS in the anterior cingulate cortex ( ACC ) , a ROI linked to focused attention , and with a shift of neuronal activation in alpha 2 band from the bilateral superior parietal areas to the homologous area of the left hemisphere .
	manualset3
112453	5	403298	5	NULL	NULL	0	NULL	anterior cingulate cortex ( ACC )	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Motor learning and movement automatization were characterized by a significant reduction of theta ERS in the anterior cingulate cortex ( ACC ) , a ROI linked to focused attention , and with a shift of neuronal activation in alpha 2 band from the bilateral superior parietal areas to the homologous area of the left hemisphere .
	manualset3
112454	6	403298	5	NULL	NULL	NULL	NULL	ROI	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Motor learning and movement automatization were characterized by a significant reduction of theta ERS in the anterior cingulate cortex ( ACC ) , a ROI linked to focused attention , and with a shift of neuronal activation in alpha 2 band from the bilateral superior parietal areas to the homologous area of the left hemisphere .
	manualset3
112455	7	403298	5	NULL	NULL	0	NULL	focused attention	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Motor learning and movement automatization were characterized by a significant reduction of theta ERS in the anterior cingulate cortex ( ACC ) , a ROI linked to focused attention , and with a shift of neuronal activation in alpha 2 band from the bilateral superior parietal areas to the homologous area of the left hemisphere .
	manualset3
112456	8	403298	5	NULL	NULL	0	NULL	neuronal activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Motor learning and movement automatization were characterized by a significant reduction of theta ERS in the anterior cingulate cortex ( ACC ) , a ROI linked to focused attention , and with a shift of neuronal activation in alpha 2 band from the bilateral superior parietal areas to the homologous area of the left hemisphere .
	manualset3
112457	9	403298	5	NULL	NULL	0	NULL	alpha 2 band	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Motor learning and movement automatization were characterized by a significant reduction of theta ERS in the anterior cingulate cortex ( ACC ) , a ROI linked to focused attention , and with a shift of neuronal activation in alpha 2 band from the bilateral superior parietal areas to the homologous area of the left hemisphere .
	manualset3
112458	10	403298	5	NULL	NULL	0	NULL	bilateral superior parietal areas	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Motor learning and movement automatization were characterized by a significant reduction of theta ERS in the anterior cingulate cortex ( ACC ) , a ROI linked to focused attention , and with a shift of neuronal activation in alpha 2 band from the bilateral superior parietal areas to the homologous area of the left hemisphere .
	manualset3
112459	11	403298	5	NULL	NULL	0	NULL	homologous area	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Motor learning and movement automatization were characterized by a significant reduction of theta ERS in the anterior cingulate cortex ( ACC ) , a ROI linked to focused attention , and with a shift of neuronal activation in alpha 2 band from the bilateral superior parietal areas to the homologous area of the left hemisphere .
	manualset3
112460	12	403298	5	NULL	NULL	0	NULL	left hemisphere	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Motor learning and movement automatization were characterized by a significant reduction of theta ERS in the anterior cingulate cortex ( ACC ) , a ROI linked to focused attention , and with a shift of neuronal activation in alpha 2 band from the bilateral superior parietal areas to the homologous area of the left hemisphere .
	manualset3
112461	1	403299	5	NULL	NULL	0	NULL	Mouse Gipc3 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Mouse Gipc3 mRNA was relatively highly expressed in adult lung , and was also expressed in brain and testis , but was almost undetectable in 7 - , 11 - , 15 , and 17-day whole embryos .
	manualset3
112462	2	403299	5	NULL	NULL	0	NULL	adult lung	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mouse Gipc3 mRNA was relatively highly expressed in adult lung , and was also expressed in brain and testis , but was almost undetectable in 7 - , 11 - , 15 , and 17-day whole embryos .
	manualset3
112463	3	403299	5	NULL	NULL	0	NULL	brain 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mouse Gipc3 mRNA was relatively highly expressed in adult lung , and was also expressed in brain and testis , but was almost undetectable in 7 - , 11 - , 15 , and 17-day whole embryos .
	manualset3
112464	4	403299	5	NULL	NULL	0	NULL	testis 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mouse Gipc3 mRNA was relatively highly expressed in adult lung , and was also expressed in brain and testis , but was almost undetectable in 7 - , 11 - , 15 , and 17-day whole embryos .
	manualset3
112465	5	403299	5	NULL	NULL	0	NULL	7 - , 11 - , 15 , and 17-day whole embryos	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mouse Gipc3 mRNA was relatively highly expressed in adult lung , and was also expressed in brain and testis , but was almost undetectable in 7 - , 11 - , 15 , and 17-day whole embryos .
	manualset3
112466	1	403300	5	NULL	NULL	0	NULL	Mouse ileal alkaline phosphatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mouse ileal alkaline phosphatase is a sialyl enzyme ( 12-14 moles per mole of enzyme ) .
	manualset3
112467	2	403300	5	NULL	NULL	0	NULL	sialyl enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mouse ileal alkaline phosphatase is a sialyl enzyme ( 12-14 moles per mole of enzyme ) .
	manualset3
112468	3	403300	5	NULL	NULL	NULL	NULL	12-14 moles per mole	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mouse ileal alkaline phosphatase is a sialyl enzyme ( 12-14 moles per mole of enzyme ) .
	manualset3
112982	4	403300	5	NULL	NULL	0	NULL	enzyme 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mouse ileal alkaline phosphatase is a sialyl enzyme ( 12-14 moles per mole of enzyme ) .
	manualset3
112469	1	403301	5	NULL	NULL	0	NULL	Mouse mammary tumor virus ( MMTV ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mouse mammary tumor virus ( MMTV ) is a B type retrovirus transmitted to the suckling offspring through milk .
	manualset3
112470	2	403301	5	NULL	NULL	0	NULL	B type retrovirus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mouse mammary tumor virus ( MMTV ) is a B type retrovirus transmitted to the suckling offspring through milk .
	manualset3
112471	3	403301	5	NULL	NULL	0	NULL	suckling offspring	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mouse mammary tumor virus ( MMTV ) is a B type retrovirus transmitted to the suckling offspring through milk .
	manualset3
112472	4	403301	5	NULL	NULL	0	NULL	milk 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Mouse mammary tumor virus ( MMTV ) is a B type retrovirus transmitted to the suckling offspring through milk .
	manualset3
112473	1	403302	5	NULL	NULL	0	NULL	Mouse models 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Mouse models have proved valuable tools in the analysis of human genetic disorders .
	manualset3
112474	2	403302	5	NULL	NULL	0	NULL	valuable tools	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Mouse models have proved valuable tools in the analysis of human genetic disorders .
	manualset3
112475	3	403302	5	NULL	NULL	0	NULL	analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mouse models have proved valuable tools in the analysis of human genetic disorders .
	manualset3
112476	4	403302	5	NULL	NULL	0	NULL	human genetic disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mouse models have proved valuable tools in the analysis of human genetic disorders .
	manualset3
112477	1	403303	5	NULL	NULL	0	NULL	Mouse models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Mouse models of transforming growth factor beta impact in breast development and cancer .
	manualset3
112478	2	403303	5	NULL	NULL	0	NULL	transforming growth factor beta 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mouse models of transforming growth factor beta impact in breast development and cancer .
	manualset3
112479	3	403303	5	NULL	NULL	0	NULL	breast development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mouse models of transforming growth factor beta impact in breast development and cancer .
	manualset3
112480	4	403303	5	NULL	NULL	0	NULL	cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mouse models of transforming growth factor beta impact in breast development and cancer .
	manualset3
112481	1	403304	5	NULL	NULL	0	NULL	Movement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Movement of meiosis I ( MI ) chromosomes from the oocyte center to a subcortical location is the first step in the establishment of cortical polarity .
	manualset3
112482	2	403304	5	NULL	NULL	0	NULL	meiosis I ( MI ) chromosomes 	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Movement of meiosis I ( MI ) chromosomes from the oocyte center to a subcortical location is the first step in the establishment of cortical polarity .
	manualset3
112483	3	403304	5	NULL	NULL	NULL	NULL	oocyte center	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Movement of meiosis I ( MI ) chromosomes from the oocyte center to a subcortical location is the first step in the establishment of cortical polarity .
	manualset3
112484	4	403304	5	NULL	NULL	0	NULL	subcortical location	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Movement of meiosis I ( MI ) chromosomes from the oocyte center to a subcortical location is the first step in the establishment of cortical polarity .
	manualset3
112485	5	403304	5	NULL	NULL	0	NULL	first step	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Movement of meiosis I ( MI ) chromosomes from the oocyte center to a subcortical location is the first step in the establishment of cortical polarity .
	manualset3
112486	6	403304	5	NULL	NULL	0	NULL	establishment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Movement of meiosis I ( MI ) chromosomes from the oocyte center to a subcortical location is the first step in the establishment of cortical polarity .
	manualset3
112487	7	403304	5	NULL	NULL	0	NULL	cortical polarity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Movement of meiosis I ( MI ) chromosomes from the oocyte center to a subcortical location is the first step in the establishment of cortical polarity .
	manualset3
112488	1	403305	5	NULL	NULL	0	NULL	Movement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Movement of the implant was a possible reason for the prolonged healing time .
	manualset3
112489	2	403305	5	NULL	NULL	0	NULL	implant 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Movement of the implant was a possible reason for the prolonged healing time .
	manualset3
112490	3	403305	5	NULL	NULL	0	NULL	possible reason 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Movement of the implant was a possible reason for the prolonged healing time .
	manualset3
112491	4	403305	5	NULL	NULL	0	NULL	prolonged healing time	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Movement of the implant was a possible reason for the prolonged healing time .
	manualset3
112492	1	403306	5	NULL	NULL	0	NULL	reason 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moving as a reason for pet relinquishment : a closer look .
	manualset3
112493	2	403306	5	NULL	NULL	0	NULL	pet relinquishment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moving as a reason for pet relinquishment : a closer look .
	manualset3
112494	1	403307	5	NULL	NULL	0	NULL	Mssbauer spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mssbauer spectroscopy of anaerobically purified HemN has identified a predominantly ( 4Fe-4S ) ( 2 + ) cluster in which only three iron atoms were coordinated by cysteine residues ( isomer shift of delta = 0.43 ( 1 ) mm/s ) .
	manualset3
112495	2	403307	5	NULL	NULL	0	NULL	anaerobically purified HemN	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mssbauer spectroscopy of anaerobically purified HemN has identified a predominantly ( 4Fe-4S ) ( 2 + ) cluster in which only three iron atoms were coordinated by cysteine residues ( isomer shift of delta = 0.43 ( 1 ) mm/s ) .
	manualset3
112496	3	403307	5	NULL	NULL	0	NULL	( 4Fe-4S ) ( 2 + ) cluster	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mssbauer spectroscopy of anaerobically purified HemN has identified a predominantly ( 4Fe-4S ) ( 2 + ) cluster in which only three iron atoms were coordinated by cysteine residues ( isomer shift of delta = 0.43 ( 1 ) mm/s ) .
	manualset3
112497	4	403307	5	NULL	NULL	0	NULL	three iron atoms	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Mssbauer spectroscopy of anaerobically purified HemN has identified a predominantly ( 4Fe-4S ) ( 2 + ) cluster in which only three iron atoms were coordinated by cysteine residues ( isomer shift of delta = 0.43 ( 1 ) mm/s ) .
	manualset3
112498	5	403307	5	NULL	NULL	NULL	NULL	cysteine residues	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mssbauer spectroscopy of anaerobically purified HemN has identified a predominantly ( 4Fe-4S ) ( 2 + ) cluster in which only three iron atoms were coordinated by cysteine residues ( isomer shift of delta = 0.43 ( 1 ) mm/s ) .
	manualset3
112499	6	403307	5	NULL	NULL	0	NULL	isomer shift of delta = 0.43 ( 1 ) mm/s	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mssbauer spectroscopy of anaerobically purified HemN has identified a predominantly ( 4Fe-4S ) ( 2 + ) cluster in which only three iron atoms were coordinated by cysteine residues ( isomer shift of delta = 0.43 ( 1 ) mm/s ) .
	manualset3
112500	1	403308	5	NULL	NULL	NULL	NULL	close correlation 	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A close correlation was observed for the pattern of metabolites found in plasma and milk .
	manualset3
112501	2	403308	5	NULL	NULL	0	NULL	pattern 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A close correlation was observed for the pattern of metabolites found in plasma and milk .
	manualset3
112502	3	403308	5	NULL	NULL	0	NULL	metabolites 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A close correlation was observed for the pattern of metabolites found in plasma and milk .
	manualset3
112503	4	403308	5	NULL	NULL	0	NULL	plasma 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A close correlation was observed for the pattern of metabolites found in plasma and milk .
	manualset3
112504	5	403308	5	NULL	NULL	0	NULL	milk 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A close correlation was observed for the pattern of metabolites found in plasma and milk .
	manualset3
112505	1	403309	5	NULL	NULL	0	NULL	MtCDH 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	MtCDH was able to produce a sufficient amount of H2O2 to decolorize the anthocyanins within 2 h .
	manualset3
112506	2	403309	5	NULL	NULL	0	NULL	sufficient amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	MtCDH was able to produce a sufficient amount of H2O2 to decolorize the anthocyanins within 2 h .
	manualset3
112507	3	403309	5	NULL	NULL	0	NULL	H2O2 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	MtCDH was able to produce a sufficient amount of H2O2 to decolorize the anthocyanins within 2 h .
	manualset3
112508	4	403309	5	NULL	NULL	0	NULL	anthocyanins 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	MtCDH was able to produce a sufficient amount of H2O2 to decolorize the anthocyanins within 2 h .
	manualset3
112509	5	403309	5	NULL	NULL	0	NULL	2 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	MtCDH was able to produce a sufficient amount of H2O2 to decolorize the anthocyanins within 2 h .
	manualset3
112510	1	403310	5	NULL	NULL	0	NULL	attention 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Much attention has been focused on DNA condensation because of its fundamental biological importance .
	manualset3
112511	2	403310	5	NULL	NULL	0	NULL	DNA condensation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Much attention has been focused on DNA condensation because of its fundamental biological importance .
	manualset3
112512	3	403310	5	NULL	NULL	0	NULL	fundamental biological importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Much attention has been focused on DNA condensation because of its fundamental biological importance .
	manualset3
112513	1	403311	5	NULL	NULL	0	NULL	effort 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Much effort has been put into development of software that deploys legacy applications on a grid-based infrastructure and efficiently uses available resources .
	manualset3
112514	2	403311	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Much effort has been put into development of software that deploys legacy applications on a grid-based infrastructure and efficiently uses available resources .
	manualset3
112515	3	403311	5	NULL	NULL	0	NULL	software 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Much effort has been put into development of software that deploys legacy applications on a grid-based infrastructure and efficiently uses available resources .
	manualset3
112516	4	403311	5	NULL	NULL	0	NULL	legacy applications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Much effort has been put into development of software that deploys legacy applications on a grid-based infrastructure and efficiently uses available resources .
	manualset3
112517	5	403311	5	NULL	NULL	0	NULL	grid-based infrastructure 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Much effort has been put into development of software that deploys legacy applications on a grid-based infrastructure and efficiently uses available resources .
	manualset3
112518	6	403311	5	NULL	NULL	0	NULL	resources 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Much effort has been put into development of software that deploys legacy applications on a grid-based infrastructure and efficiently uses available resources .
	manualset3
112519	1	403312	5	NULL	NULL	0	NULL	INFOODS 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Much has been accomplished by INFOODS , despite limited resources .
	manualset3
112520	2	403312	5	NULL	NULL	0	NULL	resources 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Much has been accomplished by INFOODS , despite limited resources .
	manualset3
112521	1	403313	5	NULL	NULL	0	NULL	mental health	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Much of the mental health , substance use , and educational programming within a particular women 's prison in the southwestern United States promotes individual choice and agency .
	manualset3
112522	2	403313	5	NULL	NULL	0	NULL	substance use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Much of the mental health , substance use , and educational programming within a particular women 's prison in the southwestern United States promotes individual choice and agency .
	manualset3
112523	3	403313	5	NULL	NULL	0	NULL	educational programming	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Much of the mental health , substance use , and educational programming within a particular women 's prison in the southwestern United States promotes individual choice and agency .
	manualset3
112524	4	403313	5	NULL	NULL	0	NULL	women 's prison	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Much of the mental health , substance use , and educational programming within a particular women 's prison in the southwestern United States promotes individual choice and agency .
	manualset3
112525	5	403313	5	NULL	NULL	0	NULL	southwestern United States 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Much of the mental health , substance use , and educational programming within a particular women 's prison in the southwestern United States promotes individual choice and agency .
	manualset3
112526	6	403313	5	NULL	NULL	0	NULL	individual choice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Much of the mental health , substance use , and educational programming within a particular women 's prison in the southwestern United States promotes individual choice and agency .
	manualset3
112527	7	403313	5	NULL	NULL	0	NULL	agency 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Much of the mental health , substance use , and educational programming within a particular women 's prison in the southwestern United States promotes individual choice and agency .
	manualset3
112528	1	403314	5	NULL	NULL	0	NULL	essentials 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Much can be learned about the essentials of nematode biology by studying C. elegans , but discovering the basic biology of nematode parasitism can only be gained through comparative studies on multiple parasitic species .
	manualset3
112529	2	403314	5	NULL	NULL	0	NULL	nematode biology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Much can be learned about the essentials of nematode biology by studying C. elegans , but discovering the basic biology of nematode parasitism can only be gained through comparative studies on multiple parasitic species .
	manualset3
112530	3	403314	5	NULL	NULL	0	NULL	C. elegans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Much can be learned about the essentials of nematode biology by studying C. elegans , but discovering the basic biology of nematode parasitism can only be gained through comparative studies on multiple parasitic species .
	manualset3
112531	4	403314	5	NULL	NULL	0	NULL	basic biology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Much can be learned about the essentials of nematode biology by studying C. elegans , but discovering the basic biology of nematode parasitism can only be gained through comparative studies on multiple parasitic species .
	manualset3
112532	5	403314	5	NULL	NULL	0	NULL	nematode parasitism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Much can be learned about the essentials of nematode biology by studying C. elegans , but discovering the basic biology of nematode parasitism can only be gained through comparative studies on multiple parasitic species .
	manualset3
112533	6	403314	5	NULL	NULL	0	NULL	comparative studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Much can be learned about the essentials of nematode biology by studying C. elegans , but discovering the basic biology of nematode parasitism can only be gained through comparative studies on multiple parasitic species .
	manualset3
112534	7	403314	5	NULL	NULL	0	NULL	multiple parasitic species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Much can be learned about the essentials of nematode biology by studying C. elegans , but discovering the basic biology of nematode parasitism can only be gained through comparative studies on multiple parasitic species .
	manualset3
112535	1	403315	5	NULL	NULL	0	NULL	Mucin secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mucin secretion was quantitated by enzyme-linked immunosorbent assay using a monoclonal antibody raised against airway mucin-type glycoproteins .
	manualset3
112536	2	403315	5	NULL	NULL	0	NULL	enzyme-linked immunosorbent assay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mucin secretion was quantitated by enzyme-linked immunosorbent assay using a monoclonal antibody raised against airway mucin-type glycoproteins .
	manualset3
112537	3	403315	5	NULL	NULL	NULL	NULL	monoclonal antibody 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mucin secretion was quantitated by enzyme-linked immunosorbent assay using a monoclonal antibody raised against airway mucin-type glycoproteins .
	manualset3
112538	4	403315	5	NULL	NULL	0	NULL	airway mucin-type glycoproteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mucin secretion was quantitated by enzyme-linked immunosorbent assay using a monoclonal antibody raised against airway mucin-type glycoproteins .
	manualset3
112539	1	403316	5	NULL	NULL	0	NULL	Mucositis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mucositis was induced with 5-fluorouracil using a standard regimen of 60 mg/kg , intraperitoneally on days 0 and 2 followed by superficial mucosal irritation on day 4 .
	manualset3
112540	2	403316	5	NULL	NULL	0	NULL	 5-fluorouracil	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Mucositis was induced with 5-fluorouracil using a standard regimen of 60 mg/kg , intraperitoneally on days 0 and 2 followed by superficial mucosal irritation on day 4 .
	manualset3
112541	3	403316	5	NULL	NULL	0	NULL	standard regimen 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Mucositis was induced with 5-fluorouracil using a standard regimen of 60 mg/kg , intraperitoneally on days 0 and 2 followed by superficial mucosal irritation on day 4 .
	manualset3
112542	4	403316	5	NULL	NULL	0	NULL	60 mg/kg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mucositis was induced with 5-fluorouracil using a standard regimen of 60 mg/kg , intraperitoneally on days 0 and 2 followed by superficial mucosal irritation on day 4 .
	manualset3
112543	5	403316	5	NULL	NULL	0	NULL	days 0 and 2	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Mucositis was induced with 5-fluorouracil using a standard regimen of 60 mg/kg , intraperitoneally on days 0 and 2 followed by superficial mucosal irritation on day 4 .
	manualset3
112544	6	403316	5	NULL	NULL	0	NULL	superficial mucosal irritation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mucositis was induced with 5-fluorouracil using a standard regimen of 60 mg/kg , intraperitoneally on days 0 and 2 followed by superficial mucosal irritation on day 4 .
	manualset3
112545	7	403316	5	NULL	NULL	0	NULL	day 4 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Mucositis was induced with 5-fluorouracil using a standard regimen of 60 mg/kg , intraperitoneally on days 0 and 2 followed by superficial mucosal irritation on day 4 .
	manualset3
112546	1	403317	5	NULL	NULL	0	NULL	close relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A close relationship was suggested between the enhancement effect on MRI and histopathology of the cyst wall .
	manualset3
112547	2	403317	5	NULL	NULL	0	NULL	enhancement effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A close relationship was suggested between the enhancement effect on MRI and histopathology of the cyst wall .
	manualset3
112548	3	403317	5	NULL	NULL	0	NULL	MRI	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A close relationship was suggested between the enhancement effect on MRI and histopathology of the cyst wall .
	manualset3
112549	4	403317	5	NULL	NULL	0	NULL	histopathology 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A close relationship was suggested between the enhancement effect on MRI and histopathology of the cyst wall .
	manualset3
112550	5	403317	5	NULL	NULL	0	NULL	cyst wall	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A close relationship was suggested between the enhancement effect on MRI and histopathology of the cyst wall .
	manualset3
112551	1	403318	5	NULL	NULL	0	NULL	Multi-assay-based structure-activity relationship models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Multi-assay-based structure-activity relationship models : improving structure-activity relationship models by incorporating activity information from related targets .
	manualset3
112552	2	403318	5	NULL	NULL	0	NULL	structure-activity relationship models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Multi-assay-based structure-activity relationship models : improving structure-activity relationship models by incorporating activity information from related targets .
	manualset3
112553	3	403318	5	NULL	NULL	0	NULL	activity information	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Multi-assay-based structure-activity relationship models : improving structure-activity relationship models by incorporating activity information from related targets .
	manualset3
112554	4	403318	5	NULL	NULL	0	NULL	targets 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multi-assay-based structure-activity relationship models : improving structure-activity relationship models by incorporating activity information from related targets .
	manualset3
112555	1	403319	5	NULL	NULL	0	NULL	Multi-professional collaboration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Multi-professional collaboration across the West Midlands has developed an online generic induction package consisting of 18 statutory , mandatory and general modules .
	manualset3
112556	2	403319	5	NULL	NULL	0	NULL	West Midlands 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Multi-professional collaboration across the West Midlands has developed an online generic induction package consisting of 18 statutory , mandatory and general modules .
	manualset3
112557	3	403319	5	NULL	NULL	0	NULL	online generic induction package	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Multi-professional collaboration across the West Midlands has developed an online generic induction package consisting of 18 statutory , mandatory and general modules .
	manualset3
112558	4	403319	5	NULL	NULL	0	NULL	18 statutory , mandatory and general modules	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multi-professional collaboration across the West Midlands has developed an online generic induction package consisting of 18 statutory , mandatory and general modules .
	manualset3
112559	1	403320	5	NULL	NULL	0	NULL	CpG island hyper-methylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Multi-step aberrant CpG island hyper-methylation is associated with the progression of adult T-cell leukemia/lymphoma .
	manualset3
112560	2	403320	5	NULL	NULL	0	NULL	progression 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Multi-step aberrant CpG island hyper-methylation is associated with the progression of adult T-cell leukemia/lymphoma .
	manualset3
112561	3	403320	5	NULL	NULL	0	NULL	adult T-cell leukemia/lymphoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Multi-step aberrant CpG island hyper-methylation is associated with the progression of adult T-cell leukemia/lymphoma .
	manualset3
112562	1	403321	5	NULL	NULL	0	NULL	Multidisciplinary audit	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Multidisciplinary audit -- who 's responsible ?
	manualset3
112563	1	403322	5	NULL	NULL	0	NULL	Ca2 + / calmodulin-dependent protein kinase type II ( CaMK II ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Multifunctional Ca2 + / calmodulin-dependent protein kinase type II ( CaMK II ) plays a crucial role in mediation of cellular responses to rising cytosolic Ca2 + levels .
	manualset3
112564	2	403322	5	NULL	NULL	0	NULL	crucial role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Multifunctional Ca2 + / calmodulin-dependent protein kinase type II ( CaMK II ) plays a crucial role in mediation of cellular responses to rising cytosolic Ca2 + levels .
	manualset3
112565	3	403322	5	NULL	NULL	0	NULL	mediation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Multifunctional Ca2 + / calmodulin-dependent protein kinase type II ( CaMK II ) plays a crucial role in mediation of cellular responses to rising cytosolic Ca2 + levels .
	manualset3
112566	4	403322	5	NULL	NULL	0	NULL	cellular responses 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Multifunctional Ca2 + / calmodulin-dependent protein kinase type II ( CaMK II ) plays a crucial role in mediation of cellular responses to rising cytosolic Ca2 + levels .
	manualset3
112567	5	403322	5	NULL	NULL	0	NULL	cytosolic Ca2 + levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multifunctional Ca2 + / calmodulin-dependent protein kinase type II ( CaMK II ) plays a crucial role in mediation of cellular responses to rising cytosolic Ca2 + levels .
	manualset3
112568	1	403323	5	NULL	NULL	0	NULL	Multigram quantities 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multigram quantities ( 2.5-10 g ) of highly purified IgG were obtained within 4 h from serum by using Avid AL packed in a radial-flow column .
	manualset3
112569	2	403323	5	NULL	NULL	0	NULL	2.5-10 g	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Multigram quantities ( 2.5-10 g ) of highly purified IgG were obtained within 4 h from serum by using Avid AL packed in a radial-flow column .
	manualset3
112570	3	403323	5	NULL	NULL	NULL	NULL	highly purified IgG	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Multigram quantities ( 2.5-10 g ) of highly purified IgG were obtained within 4 h from serum by using Avid AL packed in a radial-flow column .
	manualset3
112571	4	403323	5	NULL	NULL	0	NULL	4 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Multigram quantities ( 2.5-10 g ) of highly purified IgG were obtained within 4 h from serum by using Avid AL packed in a radial-flow column .
	manualset3
112572	5	403323	5	NULL	NULL	0	NULL	serum 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Multigram quantities ( 2.5-10 g ) of highly purified IgG were obtained within 4 h from serum by using Avid AL packed in a radial-flow column .
	manualset3
112573	6	403323	5	NULL	NULL	0	NULL	Avid AL	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Multigram quantities ( 2.5-10 g ) of highly purified IgG were obtained within 4 h from serum by using Avid AL packed in a radial-flow column .
	manualset3
112574	7	403323	5	NULL	NULL	0	NULL	radial-flow column	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Multigram quantities ( 2.5-10 g ) of highly purified IgG were obtained within 4 h from serum by using Avid AL packed in a radial-flow column .
	manualset3
112575	1	403324	5	NULL	NULL	0	NULL	Multimodality treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Multimodality treatment in anaplastic giant cell thyroid carcinoma .
	manualset3
112576	2	403324	5	NULL	NULL	0	NULL	anaplastic giant cell thyroid carcinoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Multimodality treatment in anaplastic giant cell thyroid carcinoma .
	manualset3
112577	1	403325	5	NULL	NULL	0	NULL	Multinomial logistic regression 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Multinomial logistic regression was used to identify demographic and health-related characteristics associated with the number of adherence to guideline recommendations .
	manualset3
112578	2	403325	5	NULL	NULL	0	NULL	demographic characteristics 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multinomial logistic regression was used to identify demographic and health-related characteristics associated with the number of adherence to guideline recommendations .
	manualset3
112579	3	403325	5	NULL	NULL	0	NULL	 health-related characteristics 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multinomial logistic regression was used to identify demographic and health-related characteristics associated with the number of adherence to guideline recommendations .
	manualset3
112580	4	403325	5	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multinomial logistic regression was used to identify demographic and health-related characteristics associated with the number of adherence to guideline recommendations .
	manualset3
112581	5	403325	5	NULL	NULL	0	NULL	adherence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Multinomial logistic regression was used to identify demographic and health-related characteristics associated with the number of adherence to guideline recommendations .
	manualset3
112582	6	403325	5	NULL	NULL	0	NULL	guideline recommendations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Multinomial logistic regression was used to identify demographic and health-related characteristics associated with the number of adherence to guideline recommendations .
	manualset3
112583	1	403326	5	NULL	NULL	0	NULL	KCNQ potassium channel subtypes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple KCNQ potassium channel subtypes mediate basal anion secretion from the human airway epithelial cell line Calu-3 .
	manualset3
112584	2	403326	5	NULL	NULL	0	NULL	basal anion secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple KCNQ potassium channel subtypes mediate basal anion secretion from the human airway epithelial cell line Calu-3 .
	manualset3
112585	3	403326	5	NULL	NULL	0	NULL	human airway epithelial cell line Calu-3	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple KCNQ potassium channel subtypes mediate basal anion secretion from the human airway epithelial cell line Calu-3 .
	manualset3
112586	1	403327	5	NULL	NULL	0	NULL	SNPs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple SNPs in sequences under evolutionary constraint within intron 5 of FHIT defined several related haplotypes with an increased risk of prostate cancer in European-Americans .
	manualset3
112587	2	403327	5	NULL	NULL	0	NULL	sequences 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple SNPs in sequences under evolutionary constraint within intron 5 of FHIT defined several related haplotypes with an increased risk of prostate cancer in European-Americans .
	manualset3
112588	3	403327	5	NULL	NULL	0	NULL	evolutionary constraint 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple SNPs in sequences under evolutionary constraint within intron 5 of FHIT defined several related haplotypes with an increased risk of prostate cancer in European-Americans .
	manualset3
112589	4	403327	5	NULL	NULL	0	NULL	intron 5	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple SNPs in sequences under evolutionary constraint within intron 5 of FHIT defined several related haplotypes with an increased risk of prostate cancer in European-Americans .
	manualset3
112590	5	403327	5	NULL	NULL	0	NULL	FHIT 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple SNPs in sequences under evolutionary constraint within intron 5 of FHIT defined several related haplotypes with an increased risk of prostate cancer in European-Americans .
	manualset3
112591	6	403327	5	NULL	NULL	0	NULL	haplotypes 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple SNPs in sequences under evolutionary constraint within intron 5 of FHIT defined several related haplotypes with an increased risk of prostate cancer in European-Americans .
	manualset3
112592	7	403327	5	NULL	NULL	0	NULL	risk 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple SNPs in sequences under evolutionary constraint within intron 5 of FHIT defined several related haplotypes with an increased risk of prostate cancer in European-Americans .
	manualset3
112593	8	403327	5	NULL	NULL	0	NULL	prostate cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple SNPs in sequences under evolutionary constraint within intron 5 of FHIT defined several related haplotypes with an increased risk of prostate cancer in European-Americans .
	manualset3
112594	9	403327	5	NULL	NULL	0	NULL	European-Americans	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple SNPs in sequences under evolutionary constraint within intron 5 of FHIT defined several related haplotypes with an increased risk of prostate cancer in European-Americans .
	manualset3
112595	1	403328	5	NULL	NULL	0	NULL	afferent pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple afferent pathways underlie the control of adrenocorticotropin ( ACTH ) .
	manualset3
112596	2	403328	5	NULL	NULL	0	NULL	control 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple afferent pathways underlie the control of adrenocorticotropin ( ACTH ) .
	manualset3
112597	3	403328	5	NULL	NULL	0	NULL	adrenocorticotropin ( ACTH ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple afferent pathways underlie the control of adrenocorticotropin ( ACTH ) .
	manualset3
112598	1	403329	5	NULL	NULL	0	NULL	Multiple alignment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple alignment of amino acid sequence revealed that a previously unidentified Cys-61 is most conserved among all bacterial p20 scavengases and corresponds to the active site in the well-characterized peroxiredoxins .
	manualset3
112599	2	403329	5	NULL	NULL	0	NULL	amino acid sequence	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple alignment of amino acid sequence revealed that a previously unidentified Cys-61 is most conserved among all bacterial p20 scavengases and corresponds to the active site in the well-characterized peroxiredoxins .
	manualset3
112600	3	403329	5	NULL	NULL	0	NULL	Cys-61	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple alignment of amino acid sequence revealed that a previously unidentified Cys-61 is most conserved among all bacterial p20 scavengases and corresponds to the active site in the well-characterized peroxiredoxins .
	manualset3
112601	4	403329	5	NULL	NULL	NULL	NULL	bacterial p20 scavengases 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Multiple alignment of amino acid sequence revealed that a previously unidentified Cys-61 is most conserved among all bacterial p20 scavengases and corresponds to the active site in the well-characterized peroxiredoxins .
	manualset3
112602	5	403329	5	NULL	NULL	0	NULL	active site 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple alignment of amino acid sequence revealed that a previously unidentified Cys-61 is most conserved among all bacterial p20 scavengases and corresponds to the active site in the well-characterized peroxiredoxins .
	manualset3
112603	6	403329	5	NULL	NULL	0	NULL	peroxiredoxins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple alignment of amino acid sequence revealed that a previously unidentified Cys-61 is most conserved among all bacterial p20 scavengases and corresponds to the active site in the well-characterized peroxiredoxins .
	manualset3
112604	1	403330	5	NULL	NULL	0	NULL	cluster analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A cluster analysis of achievement test scores yielded 10 groups ; 6 of which met our criterion for academic deficiency .
	manualset3
112605	2	403330	5	NULL	NULL	0	NULL	achievement test scores	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A cluster analysis of achievement test scores yielded 10 groups ; 6 of which met our criterion for academic deficiency .
	manualset3
112606	3	403330	5	NULL	NULL	0	NULL	10 groups 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A cluster analysis of achievement test scores yielded 10 groups ; 6 of which met our criterion for academic deficiency .
	manualset3
112607	4	403330	5	NULL	NULL	0	NULL	6	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A cluster analysis of achievement test scores yielded 10 groups ; 6 of which met our criterion for academic deficiency .
	manualset3
112608	5	403330	5	NULL	NULL	0	NULL	criterion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A cluster analysis of achievement test scores yielded 10 groups ; 6 of which met our criterion for academic deficiency .
	manualset3
112609	6	403330	5	NULL	NULL	0	NULL	academic deficiency 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A cluster analysis of achievement test scores yielded 10 groups ; 6 of which met our criterion for academic deficiency .
	manualset3
112736	1	403331	5	NULL	NULL	0	NULL	Multiple displacement amplification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple displacement amplification for preimplantation genetic diagnosis of fragile X syndrome .
	manualset3
112737	2	403331	5	NULL	NULL	NULL	NULL	preimplantation genetic diagnosis	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Multiple displacement amplification for preimplantation genetic diagnosis of fragile X syndrome .
	manualset3
112738	3	403331	5	NULL	NULL	0	NULL	fragile X syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple displacement amplification for preimplantation genetic diagnosis of fragile X syndrome .
	manualset3
112739	1	403332	5	NULL	NULL	0	NULL	Multiple episodes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple episodes of ischemic preconditioning are not associated with loss of benefit : preliminary clinical experience .
	manualset3
112740	2	403332	5	NULL	NULL	0	NULL	ischemic preconditioning	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple episodes of ischemic preconditioning are not associated with loss of benefit : preliminary clinical experience .
	manualset3
112741	3	403332	5	NULL	NULL	0	NULL	loss 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple episodes of ischemic preconditioning are not associated with loss of benefit : preliminary clinical experience .
	manualset3
112742	4	403332	5	NULL	NULL	0	NULL	benefit 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple episodes of ischemic preconditioning are not associated with loss of benefit : preliminary clinical experience .
	manualset3
112743	5	403332	5	NULL	NULL	0	NULL	preliminary clinical experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple episodes of ischemic preconditioning are not associated with loss of benefit : preliminary clinical experience .
	manualset3
112744	1	403333	5	NULL	NULL	0	NULL	Multiple factors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple factors confer specific Cdc42 and Rac protein activation by dedicator of cytokinesis ( DOCK ) nucleotide exchange factors .
	manualset3
112745	2	403333	5	NULL	NULL	0	NULL	Cdc42 protein activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple factors confer specific Cdc42 and Rac protein activation by dedicator of cytokinesis ( DOCK ) nucleotide exchange factors .
	manualset3
112746	3	403333	5	NULL	NULL	0	NULL	Rac protein activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple factors confer specific Cdc42 and Rac protein activation by dedicator of cytokinesis ( DOCK ) nucleotide exchange factors .
	manualset3
112747	4	403333	5	NULL	NULL	NULL	NULL	dedicator of cytokinesis ( DOCK ) nucleotide exchange factors 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Multiple factors confer specific Cdc42 and Rac protein activation by dedicator of cytokinesis ( DOCK ) nucleotide exchange factors .
	manualset3
112748	1	403334	5	NULL	NULL	0	NULL	insulin injections 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple insulin injections using an injection pen are acceptable to adolescent diabetics and improve their control .
	manualset3
112749	2	403334	5	NULL	NULL	0	NULL	injection pen	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple insulin injections using an injection pen are acceptable to adolescent diabetics and improve their control .
	manualset3
112750	3	403334	5	NULL	NULL	0	NULL	adolescent diabetics	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple insulin injections using an injection pen are acceptable to adolescent diabetics and improve their control .
	manualset3
112751	4	403334	5	NULL	NULL	0	NULL	control 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple insulin injections using an injection pen are acceptable to adolescent diabetics and improve their control .
	manualset3
112752	1	403335	5	NULL	NULL	0	NULL	levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple levels of regulation of protein synthesis at fertilization in sea urchin eggs .
	manualset3
112753	2	403335	5	NULL	NULL	0	NULL	regulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple levels of regulation of protein synthesis at fertilization in sea urchin eggs .
	manualset3
112754	3	403335	5	NULL	NULL	0	NULL	protein synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple levels of regulation of protein synthesis at fertilization in sea urchin eggs .
	manualset3
112755	4	403335	5	NULL	NULL	0	NULL	fertilization 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple levels of regulation of protein synthesis at fertilization in sea urchin eggs .
	manualset3
112756	5	403335	5	NULL	NULL	0	NULL	sea urchin eggs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple levels of regulation of protein synthesis at fertilization in sea urchin eggs .
	manualset3
112757	1	403336	5	NULL	NULL	0	NULL	Multiple myeloma ( MM )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple myeloma ( MM ) , a B-cell malignancy characterized by proliferation of monoclonal plasma cells remains incurable .
	manualset3
112758	2	403336	5	NULL	NULL	0	NULL	B-cell malignancy 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple myeloma ( MM ) , a B-cell malignancy characterized by proliferation of monoclonal plasma cells remains incurable .
	manualset3
112759	3	403336	5	NULL	NULL	0	NULL	proliferation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple myeloma ( MM ) , a B-cell malignancy characterized by proliferation of monoclonal plasma cells remains incurable .
	manualset3
112760	4	403336	5	NULL	NULL	0	NULL	monoclonal plasma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple myeloma ( MM ) , a B-cell malignancy characterized by proliferation of monoclonal plasma cells remains incurable .
	manualset3
112761	1	403337	5	NULL	NULL	0	NULL	coalition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A coalition of 49 AIDS organizations and civil rights groups are fighting an `` aggressive push '' by the Centers for Disease Control and Prevention ( CDC ) to institute name-based HIV case surveillance .
	manualset3
112762	2	403337	5	NULL	NULL	0	NULL	49	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A coalition of 49 AIDS organizations and civil rights groups are fighting an `` aggressive push '' by the Centers for Disease Control and Prevention ( CDC ) to institute name-based HIV case surveillance .
	manualset3
112763	3	403337	5	NULL	NULL	0	NULL	AIDS organizations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A coalition of 49 AIDS organizations and civil rights groups are fighting an `` aggressive push '' by the Centers for Disease Control and Prevention ( CDC ) to institute name-based HIV case surveillance .
	manualset3
112764	4	403337	5	NULL	NULL	0	NULL	civil rights groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A coalition of 49 AIDS organizations and civil rights groups are fighting an `` aggressive push '' by the Centers for Disease Control and Prevention ( CDC ) to institute name-based HIV case surveillance .
	manualset3
112765	5	403337	5	NULL	NULL	0	NULL	Centers for Disease Control and Prevention ( CDC )	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A coalition of 49 AIDS organizations and civil rights groups are fighting an `` aggressive push '' by the Centers for Disease Control and Prevention ( CDC ) to institute name-based HIV case surveillance .
	manualset3
112766	6	403337	5	NULL	NULL	NULL	NULL	name-based HIV case surveillance	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A coalition of 49 AIDS organizations and civil rights groups are fighting an `` aggressive push '' by the Centers for Disease Control and Prevention ( CDC ) to institute name-based HIV case surveillance .
	manualset3
112767	1	403338	5	NULL	NULL	0	NULL	Multiple proteolytic pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple proteolytic pathways are involved in the degradation of the cyclin-dependent kinase inhibitor p21 ( Cip1/WAF1 ) .
	manualset3
112768	2	403338	5	NULL	NULL	0	NULL	degradation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple proteolytic pathways are involved in the degradation of the cyclin-dependent kinase inhibitor p21 ( Cip1/WAF1 ) .
	manualset3
112769	3	403338	5	NULL	NULL	0	NULL	cyclin-dependent kinase inhibitor p21 ( Cip1/WAF1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple proteolytic pathways are involved in the degradation of the cyclin-dependent kinase inhibitor p21 ( Cip1/WAF1 ) .
	manualset3
112770	1	403339	5	NULL	NULL	0	NULL	Multiple regression analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple regression analysis found infection to be associated significantly with increasing APR DRG severity , longer procedures , younger age , and male gender ( p & lt ; 0.01 for each except p = 0.02 for age ) , as well as agent choice .
	manualset3
112771	2	403339	5	NULL	NULL	0	NULL	infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple regression analysis found infection to be associated significantly with increasing APR DRG severity , longer procedures , younger age , and male gender ( p & lt ; 0.01 for each except p = 0.02 for age ) , as well as agent choice .
	manualset3
112772	3	403339	5	NULL	NULL	0	NULL	APR DRG severity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple regression analysis found infection to be associated significantly with increasing APR DRG severity , longer procedures , younger age , and male gender ( p & lt ; 0.01 for each except p = 0.02 for age ) , as well as agent choice .
	manualset3
112773	4	403339	5	NULL	NULL	0	NULL	longer procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple regression analysis found infection to be associated significantly with increasing APR DRG severity , longer procedures , younger age , and male gender ( p & lt ; 0.01 for each except p = 0.02 for age ) , as well as agent choice .
	manualset3
112774	5	403339	5	NULL	NULL	0	NULL	younger age 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple regression analysis found infection to be associated significantly with increasing APR DRG severity , longer procedures , younger age , and male gender ( p & lt ; 0.01 for each except p = 0.02 for age ) , as well as agent choice .
	manualset3
112775	6	403339	5	NULL	NULL	0	NULL	male gender 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple regression analysis found infection to be associated significantly with increasing APR DRG severity , longer procedures , younger age , and male gender ( p & lt ; 0.01 for each except p = 0.02 for age ) , as well as agent choice .
	manualset3
112776	7	403339	5	NULL	NULL	0	NULL	p & lt ; 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple regression analysis found infection to be associated significantly with increasing APR DRG severity , longer procedures , younger age , and male gender ( p & lt ; 0.01 for each except p = 0.02 for age ) , as well as agent choice .
	manualset3
112777	8	403339	5	NULL	NULL	0	NULL	p = 0.02	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple regression analysis found infection to be associated significantly with increasing APR DRG severity , longer procedures , younger age , and male gender ( p & lt ; 0.01 for each except p = 0.02 for age ) , as well as agent choice .
	manualset3
112778	9	403339	5	NULL	NULL	0	NULL	age	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple regression analysis found infection to be associated significantly with increasing APR DRG severity , longer procedures , younger age , and male gender ( p & lt ; 0.01 for each except p = 0.02 for age ) , as well as agent choice .
	manualset3
112779	10	403339	5	NULL	NULL	0	NULL	agent choice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple regression analysis found infection to be associated significantly with increasing APR DRG severity , longer procedures , younger age , and male gender ( p & lt ; 0.01 for each except p = 0.02 for age ) , as well as agent choice .
	manualset3
112780	1	403340	5	NULL	NULL	0	NULL	Multiple regression analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple regression analysis showed that both PME ( partial r = -0.29 , & lt ; 0.02 ) and ANGLY ( partial r = -0.24 , P & lt ; 0.04 ) were independently related to ARTE .
	manualset3
112781	2	403340	5	NULL	NULL	0	NULL	PME 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple regression analysis showed that both PME ( partial r = -0.29 , & lt ; 0.02 ) and ANGLY ( partial r = -0.24 , P & lt ; 0.04 ) were independently related to ARTE .
	manualset3
112782	3	403340	5	NULL	NULL	0	NULL	partial r = -0.29 , & lt ; 0.02	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple regression analysis showed that both PME ( partial r = -0.29 , & lt ; 0.02 ) and ANGLY ( partial r = -0.24 , P & lt ; 0.04 ) were independently related to ARTE .
	manualset3
112783	4	403340	5	NULL	NULL	0	NULL	ANGLY 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple regression analysis showed that both PME ( partial r = -0.29 , & lt ; 0.02 ) and ANGLY ( partial r = -0.24 , P & lt ; 0.04 ) were independently related to ARTE .
	manualset3
112784	5	403340	5	NULL	NULL	0	NULL	partial r = -0.24 , P & lt ; 0.04 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple regression analysis showed that both PME ( partial r = -0.29 , & lt ; 0.02 ) and ANGLY ( partial r = -0.24 , P & lt ; 0.04 ) were independently related to ARTE .
	manualset3
112785	6	403340	5	NULL	NULL	0	NULL	ARTE 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple regression analysis showed that both PME ( partial r = -0.29 , & lt ; 0.02 ) and ANGLY ( partial r = -0.24 , P & lt ; 0.04 ) were independently related to ARTE .
	manualset3
112786	1	403341	5	NULL	NULL	0	NULL	Multiple sclerosis ( MS )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple sclerosis ( MS ) has long been known to be associated with Leber 's hereditary optic neuropathy ( LHON ) , a disease caused by mitochondrial DNA ( mtDNA ) mutations .
	manualset3
112787	2	403341	5	NULL	NULL	0	NULL	Leber 's hereditary optic neuropathy ( LHON )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple sclerosis ( MS ) has long been known to be associated with Leber 's hereditary optic neuropathy ( LHON ) , a disease caused by mitochondrial DNA ( mtDNA ) mutations .
	manualset3
112788	3	403341	5	NULL	NULL	0	NULL	disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple sclerosis ( MS ) has long been known to be associated with Leber 's hereditary optic neuropathy ( LHON ) , a disease caused by mitochondrial DNA ( mtDNA ) mutations .
	manualset3
112789	4	403341	5	NULL	NULL	0	NULL	mitochondrial DNA ( mtDNA ) mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple sclerosis ( MS ) has long been known to be associated with Leber 's hereditary optic neuropathy ( LHON ) , a disease caused by mitochondrial DNA ( mtDNA ) mutations .
	manualset3
112790	1	403342	5	NULL	NULL	0	NULL	Multiple units	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple units in brain stem and forebrain during the first week of life in the rat .
	manualset3
112791	2	403342	5	NULL	NULL	0	NULL	brain stem	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple units in brain stem and forebrain during the first week of life in the rat .
	manualset3
112792	3	403342	5	NULL	NULL	0	NULL	forebrain 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple units in brain stem and forebrain during the first week of life in the rat .
	manualset3
112793	4	403342	5	NULL	NULL	0	NULL	first week 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple units in brain stem and forebrain during the first week of life in the rat .
	manualset3
112794	5	403342	5	NULL	NULL	0	NULL	life 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple units in brain stem and forebrain during the first week of life in the rat .
	manualset3
112795	6	403342	5	NULL	NULL	0	NULL	rat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple units in brain stem and forebrain during the first week of life in the rat .
	manualset3
112796	1	403343	5	NULL	NULL	0	NULL	Multiple zinc binding sites 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple zinc binding sites in retinal rod cGMP phosphodiesterase , PDE6alpha beta .
	manualset3
112797	2	403343	5	NULL	NULL	0	NULL	retinal rod	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple zinc binding sites in retinal rod cGMP phosphodiesterase , PDE6alpha beta .
	manualset3
112798	3	403343	5	NULL	NULL	0	NULL	cGMP phosphodiesterase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple zinc binding sites in retinal rod cGMP phosphodiesterase , PDE6alpha beta .
	manualset3
112799	4	403343	5	NULL	NULL	0	NULL	PDE6alpha beta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple zinc binding sites in retinal rod cGMP phosphodiesterase , PDE6alpha beta .
	manualset3
112800	1	403344	5	NULL	NULL	NULL	NULL	Bile flow 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Bile flow and pancreas secretion ) .
	manualset3
112801	2	403344	5	NULL	NULL	0	NULL	pancreas secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Bile flow and pancreas secretion ) .
	manualset3
112802	1	403345	5	NULL	NULL	0	NULL	coarse-grained model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A coarse-grained model is used to study the conformational properties of semiflexible polymers with amphiphilic monomer units containing both hydrophilic and hydrophobic interaction sites .
	manualset3
112804	3	403345	5	NULL	NULL	0	NULL	conformational properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A coarse-grained model is used to study the conformational properties of semiflexible polymers with amphiphilic monomer units containing both hydrophilic and hydrophobic interaction sites .
	manualset3
112805	4	403345	5	NULL	NULL	0	NULL	semiflexible polymers	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A coarse-grained model is used to study the conformational properties of semiflexible polymers with amphiphilic monomer units containing both hydrophilic and hydrophobic interaction sites .
	manualset3
112806	5	403345	5	NULL	NULL	0	NULL	amphiphilic monomer units	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A coarse-grained model is used to study the conformational properties of semiflexible polymers with amphiphilic monomer units containing both hydrophilic and hydrophobic interaction sites .
	manualset3
112807	6	403345	5	NULL	NULL	NULL	NULL	hydrophilic interaction sites	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A coarse-grained model is used to study the conformational properties of semiflexible polymers with amphiphilic monomer units containing both hydrophilic and hydrophobic interaction sites .
	manualset3
112808	7	403345	5	NULL	NULL	0	NULL	hydrophobic interaction sites	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A coarse-grained model is used to study the conformational properties of semiflexible polymers with amphiphilic monomer units containing both hydrophilic and hydrophobic interaction sites .
	manualset3
113122	1	403346	5	NULL	NULL	NULL	NULL	Multivariable logistic regression	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Multivariable logistic regression was used to assess the relationship of clinical and radiographic variables to the etiology of PN in a retrospectively identified cohort of SOT recipients at a single transplant center .
	manualset3
113123	2	403346	5	NULL	NULL	0	NULL	relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariable logistic regression was used to assess the relationship of clinical and radiographic variables to the etiology of PN in a retrospectively identified cohort of SOT recipients at a single transplant center .
	manualset3
113124	3	403346	5	NULL	NULL	0	NULL	clinical variables	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariable logistic regression was used to assess the relationship of clinical and radiographic variables to the etiology of PN in a retrospectively identified cohort of SOT recipients at a single transplant center .
	manualset3
113125	4	403346	5	NULL	NULL	0	NULL	radiographic variables	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariable logistic regression was used to assess the relationship of clinical and radiographic variables to the etiology of PN in a retrospectively identified cohort of SOT recipients at a single transplant center .
	manualset3
113126	5	403346	5	NULL	NULL	0	NULL	etiology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariable logistic regression was used to assess the relationship of clinical and radiographic variables to the etiology of PN in a retrospectively identified cohort of SOT recipients at a single transplant center .
	manualset3
113127	6	403346	5	NULL	NULL	0	NULL	PN 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariable logistic regression was used to assess the relationship of clinical and radiographic variables to the etiology of PN in a retrospectively identified cohort of SOT recipients at a single transplant center .
	manualset3
113128	7	403346	5	NULL	NULL	0	NULL	cohort 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariable logistic regression was used to assess the relationship of clinical and radiographic variables to the etiology of PN in a retrospectively identified cohort of SOT recipients at a single transplant center .
	manualset3
113129	8	403346	5	NULL	NULL	0	NULL	SOT recipients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariable logistic regression was used to assess the relationship of clinical and radiographic variables to the etiology of PN in a retrospectively identified cohort of SOT recipients at a single transplant center .
	manualset3
113130	9	403346	5	NULL	NULL	0	NULL	single transplant center	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariable logistic regression was used to assess the relationship of clinical and radiographic variables to the etiology of PN in a retrospectively identified cohort of SOT recipients at a single transplant center .
	manualset3
113131	1	403347	5	NULL	NULL	0	NULL	Multivariate analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analyses of cumulative risk of dying and time to death suggest that the major IHD risk factors are predictors of all-cause and IHD mortality in black males .
	manualset3
113132	2	403347	5	NULL	NULL	0	NULL	cumulative risk 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analyses of cumulative risk of dying and time to death suggest that the major IHD risk factors are predictors of all-cause and IHD mortality in black males .
	manualset3
113133	3	403347	5	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analyses of cumulative risk of dying and time to death suggest that the major IHD risk factors are predictors of all-cause and IHD mortality in black males .
	manualset3
113134	4	403347	5	NULL	NULL	0	NULL	death 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analyses of cumulative risk of dying and time to death suggest that the major IHD risk factors are predictors of all-cause and IHD mortality in black males .
	manualset3
113135	5	403347	5	NULL	NULL	0	NULL	IHD risk factors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analyses of cumulative risk of dying and time to death suggest that the major IHD risk factors are predictors of all-cause and IHD mortality in black males .
	manualset3
113136	6	403347	5	NULL	NULL	0	NULL	predictors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analyses of cumulative risk of dying and time to death suggest that the major IHD risk factors are predictors of all-cause and IHD mortality in black males .
	manualset3
113137	7	403347	5	NULL	NULL	0	NULL	IHD mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analyses of cumulative risk of dying and time to death suggest that the major IHD risk factors are predictors of all-cause and IHD mortality in black males .
	manualset3
113138	8	403347	5	NULL	NULL	0	NULL	black males	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analyses of cumulative risk of dying and time to death suggest that the major IHD risk factors are predictors of all-cause and IHD mortality in black males .
	manualset3
113139	1	403348	5	NULL	NULL	0	NULL	Multivariate analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis identified neither the PT nor the LNM response alone as an independent prognostic factor ; however the combined PT/LNM response was identified as an independent prognostic factor ( hazard ratio ( HR ) 2.861 , P = 0.0255 ) in addition to the number of histological lymph node metastases ( HR 2.551 , P = 0.0328 ) .
	manualset3
113284	2	403348	5	NULL	NULL	0	NULL	PT 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis identified neither the PT nor the LNM response alone as an independent prognostic factor ; however the combined PT/LNM response was identified as an independent prognostic factor ( hazard ratio ( HR ) 2.861 , P = 0.0255 ) in addition to the number of histological lymph node metastases ( HR 2.551 , P = 0.0328 ) .
	manualset3
113285	3	403348	5	NULL	NULL	0	NULL	LNM response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis identified neither the PT nor the LNM response alone as an independent prognostic factor ; however the combined PT/LNM response was identified as an independent prognostic factor ( hazard ratio ( HR ) 2.861 , P = 0.0255 ) in addition to the number of histological lymph node metastases ( HR 2.551 , P = 0.0328 ) .
	manualset3
113286	4	403348	5	NULL	NULL	NULL	NULL	independent prognostic factor	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Multivariate analysis identified neither the PT nor the LNM response alone as an independent prognostic factor ; however the combined PT/LNM response was identified as an independent prognostic factor ( hazard ratio ( HR ) 2.861 , P = 0.0255 ) in addition to the number of histological lymph node metastases ( HR 2.551 , P = 0.0328 ) .
	manualset3
113287	5	403348	5	NULL	NULL	0	NULL	combined PT/LNM response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis identified neither the PT nor the LNM response alone as an independent prognostic factor ; however the combined PT/LNM response was identified as an independent prognostic factor ( hazard ratio ( HR ) 2.861 , P = 0.0255 ) in addition to the number of histological lymph node metastases ( HR 2.551 , P = 0.0328 ) .
	manualset3
113288	6	403348	5	NULL	NULL	0	NULL	independent prognostic factor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis identified neither the PT nor the LNM response alone as an independent prognostic factor ; however the combined PT/LNM response was identified as an independent prognostic factor ( hazard ratio ( HR ) 2.861 , P = 0.0255 ) in addition to the number of histological lymph node metastases ( HR 2.551 , P = 0.0328 ) .
	manualset3
113289	7	403348	5	NULL	NULL	NULL	NULL	 hazard ratio ( HR ) 2.861 , P = 0.0255 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Multivariate analysis identified neither the PT nor the LNM response alone as an independent prognostic factor ; however the combined PT/LNM response was identified as an independent prognostic factor ( hazard ratio ( HR ) 2.861 , P = 0.0255 ) in addition to the number of histological lymph node metastases ( HR 2.551 , P = 0.0328 ) .
	manualset3
113290	8	403348	5	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis identified neither the PT nor the LNM response alone as an independent prognostic factor ; however the combined PT/LNM response was identified as an independent prognostic factor ( hazard ratio ( HR ) 2.861 , P = 0.0255 ) in addition to the number of histological lymph node metastases ( HR 2.551 , P = 0.0328 ) .
	manualset3
113291	9	403348	5	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis identified neither the PT nor the LNM response alone as an independent prognostic factor ; however the combined PT/LNM response was identified as an independent prognostic factor ( hazard ratio ( HR ) 2.861 , P = 0.0255 ) in addition to the number of histological lymph node metastases ( HR 2.551 , P = 0.0328 ) .
	manualset3
113292	10	403348	5	NULL	NULL	0	NULL	histological lymph node metastases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis identified neither the PT nor the LNM response alone as an independent prognostic factor ; however the combined PT/LNM response was identified as an independent prognostic factor ( hazard ratio ( HR ) 2.861 , P = 0.0255 ) in addition to the number of histological lymph node metastases ( HR 2.551 , P = 0.0328 ) .
	manualset3
113293	11	403348	5	NULL	NULL	0	NULL	HR 2.551 , P = 0.0328	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis identified neither the PT nor the LNM response alone as an independent prognostic factor ; however the combined PT/LNM response was identified as an independent prognostic factor ( hazard ratio ( HR ) 2.861 , P = 0.0255 ) in addition to the number of histological lymph node metastases ( HR 2.551 , P = 0.0328 ) .
	manualset3
113294	1	403349	5	NULL	NULL	0	NULL	Multivariate analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis of variance , testing for differences by age , sex , and ethnic/racial group , were applied to percentages of food matches , intrusions , and omissions between reports on the ASA24 and the interviewer-administered 24-hour diet recall .
	manualset3
113295	2	403349	5	NULL	NULL	NULL	NULL	variance 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Multivariate analysis of variance , testing for differences by age , sex , and ethnic/racial group , were applied to percentages of food matches , intrusions , and omissions between reports on the ASA24 and the interviewer-administered 24-hour diet recall .
	manualset3
113296	3	403349	5	NULL	NULL	0	NULL	age 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis of variance , testing for differences by age , sex , and ethnic/racial group , were applied to percentages of food matches , intrusions , and omissions between reports on the ASA24 and the interviewer-administered 24-hour diet recall .
	manualset3
113297	4	403349	5	NULL	NULL	0	NULL	sex 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis of variance , testing for differences by age , sex , and ethnic/racial group , were applied to percentages of food matches , intrusions , and omissions between reports on the ASA24 and the interviewer-administered 24-hour diet recall .
	manualset3
113298	5	403349	5	NULL	NULL	0	NULL	ethnic/racial group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis of variance , testing for differences by age , sex , and ethnic/racial group , were applied to percentages of food matches , intrusions , and omissions between reports on the ASA24 and the interviewer-administered 24-hour diet recall .
	manualset3
113299	6	403349	5	NULL	NULL	0	NULL	percentages 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis of variance , testing for differences by age , sex , and ethnic/racial group , were applied to percentages of food matches , intrusions , and omissions between reports on the ASA24 and the interviewer-administered 24-hour diet recall .
	manualset3
113300	7	403349	5	NULL	NULL	0	NULL	food matches	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis of variance , testing for differences by age , sex , and ethnic/racial group , were applied to percentages of food matches , intrusions , and omissions between reports on the ASA24 and the interviewer-administered 24-hour diet recall .
	manualset3
113301	8	403349	5	NULL	NULL	0	NULL	intrusions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis of variance , testing for differences by age , sex , and ethnic/racial group , were applied to percentages of food matches , intrusions , and omissions between reports on the ASA24 and the interviewer-administered 24-hour diet recall .
	manualset3
113302	9	403349	5	NULL	NULL	0	NULL	omissions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis of variance , testing for differences by age , sex , and ethnic/racial group , were applied to percentages of food matches , intrusions , and omissions between reports on the ASA24 and the interviewer-administered 24-hour diet recall .
	manualset3
113303	10	403349	5	NULL	NULL	0	NULL	reports 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis of variance , testing for differences by age , sex , and ethnic/racial group , were applied to percentages of food matches , intrusions , and omissions between reports on the ASA24 and the interviewer-administered 24-hour diet recall .
	manualset3
113304	11	403349	5	NULL	NULL	0	NULL	ASA24 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis of variance , testing for differences by age , sex , and ethnic/racial group , were applied to percentages of food matches , intrusions , and omissions between reports on the ASA24 and the interviewer-administered 24-hour diet recall .
	manualset3
113305	12	403349	5	NULL	NULL	0	NULL	interviewer-administered 24-hour diet recall	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis of variance , testing for differences by age , sex , and ethnic/racial group , were applied to percentages of food matches , intrusions , and omissions between reports on the ASA24 and the interviewer-administered 24-hour diet recall .
	manualset3
113306	1	403350	5	NULL	NULL	0	NULL	Multivariate analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis revealed that AF contributed only 1 to 1.5 days to the LOS .
	manualset3
113307	2	403350	5	NULL	NULL	0	NULL	AF 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis revealed that AF contributed only 1 to 1.5 days to the LOS .
	manualset3
113308	3	403350	5	NULL	NULL	0	NULL	1 to 1.5 days 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis revealed that AF contributed only 1 to 1.5 days to the LOS .
	manualset3
113309	4	403350	5	NULL	NULL	0	NULL	 LOS	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis revealed that AF contributed only 1 to 1.5 days to the LOS .
	manualset3
113310	1	403351	5	NULL	NULL	0	NULL	Multivariate analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis using the stepwise Cox proportional hazard model showed that lymph node metastasis was related to poor survival rates ; in addition , patients with loss of Fhit expression still tended to have poor survival ( P = 0.0563 ) .
	manualset3
113311	2	403351	5	NULL	NULL	0	NULL	stepwise Cox proportional hazard model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis using the stepwise Cox proportional hazard model showed that lymph node metastasis was related to poor survival rates ; in addition , patients with loss of Fhit expression still tended to have poor survival ( P = 0.0563 ) .
	manualset3
113312	3	403351	5	NULL	NULL	0	NULL	lymph node metastasis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis using the stepwise Cox proportional hazard model showed that lymph node metastasis was related to poor survival rates ; in addition , patients with loss of Fhit expression still tended to have poor survival ( P = 0.0563 ) .
	manualset3
113313	4	403351	5	NULL	NULL	0	NULL	poor survival rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis using the stepwise Cox proportional hazard model showed that lymph node metastasis was related to poor survival rates ; in addition , patients with loss of Fhit expression still tended to have poor survival ( P = 0.0563 ) .
	manualset3
113314	5	403351	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis using the stepwise Cox proportional hazard model showed that lymph node metastasis was related to poor survival rates ; in addition , patients with loss of Fhit expression still tended to have poor survival ( P = 0.0563 ) .
	manualset3
113315	6	403351	5	NULL	NULL	0	NULL	loss 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis using the stepwise Cox proportional hazard model showed that lymph node metastasis was related to poor survival rates ; in addition , patients with loss of Fhit expression still tended to have poor survival ( P = 0.0563 ) .
	manualset3
113316	7	403351	5	NULL	NULL	0	NULL	Fhit expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis using the stepwise Cox proportional hazard model showed that lymph node metastasis was related to poor survival rates ; in addition , patients with loss of Fhit expression still tended to have poor survival ( P = 0.0563 ) .
	manualset3
113317	8	403351	5	NULL	NULL	0	NULL	poor survival	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis using the stepwise Cox proportional hazard model showed that lymph node metastasis was related to poor survival rates ; in addition , patients with loss of Fhit expression still tended to have poor survival ( P = 0.0563 ) .
	manualset3
113318	9	403351	5	NULL	NULL	0	NULL	P = 0.0563 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Multivariate analysis using the stepwise Cox proportional hazard model showed that lymph node metastasis was related to poor survival rates ; in addition , patients with loss of Fhit expression still tended to have poor survival ( P = 0.0563 ) .
	manualset3
113319	1	403352	5	NULL	NULL	NULL	NULL	Munsell color chips 5R-5/6	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Munsell color chips 5R - , 5G - , 5B-5 / 6 , and N-5 are used as background color .
	manualset3
113320	2	403352	5	NULL	NULL	0	NULL	Munsell color chips 5G-5/6	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Munsell color chips 5R - , 5G - , 5B-5 / 6 , and N-5 are used as background color .
	manualset3
113321	3	403352	5	NULL	NULL	0	NULL	Munsell color chips 5B-5 / 6	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Munsell color chips 5R - , 5G - , 5B-5 / 6 , and N-5 are used as background color .
	manualset3
113322	4	403352	5	NULL	NULL	0	NULL	Munsell color chips N-5	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Munsell color chips 5R - , 5G - , 5B-5 / 6 , and N-5 are used as background color .
	manualset3
113323	5	403352	5	NULL	NULL	0	NULL	background color	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Munsell color chips 5R - , 5G - , 5B-5 / 6 , and N-5 are used as background color .
	manualset3
113324	1	403353	5	NULL	NULL	0	NULL	cognitive-behavioral return-to-work program	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A cognitive-behavioral return-to-work program : effects on pain patients with a history of long-term versus short-term sick leave .
	manualset3
113325	2	403353	5	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A cognitive-behavioral return-to-work program : effects on pain patients with a history of long-term versus short-term sick leave .
	manualset3
113326	3	403353	5	NULL	NULL	0	NULL	pain patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A cognitive-behavioral return-to-work program : effects on pain patients with a history of long-term versus short-term sick leave .
	manualset3
113327	4	403353	5	NULL	NULL	NULL	NULL	history 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A cognitive-behavioral return-to-work program : effects on pain patients with a history of long-term versus short-term sick leave .
	manualset3
113328	5	403353	5	NULL	NULL	0	NULL	long-term versus short-term sick leave	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A cognitive-behavioral return-to-work program : effects on pain patients with a history of long-term versus short-term sick leave .
	manualset3
113329	1	403354	5	NULL	NULL	0	NULL	MurC synthetase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	MurC and MurD synthetases of peptidoglycan biosynthesis : borohydride trapping of acyl-phosphate intermediates .
	manualset3
113330	2	403354	5	NULL	NULL	0	NULL	MurD synthetase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	MurC and MurD synthetases of peptidoglycan biosynthesis : borohydride trapping of acyl-phosphate intermediates .
	manualset3
113331	3	403354	5	NULL	NULL	0	NULL	peptidoglycan biosynthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MurC and MurD synthetases of peptidoglycan biosynthesis : borohydride trapping of acyl-phosphate intermediates .
	manualset3
113332	4	403354	5	NULL	NULL	0	NULL	borohydride 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	MurC and MurD synthetases of peptidoglycan biosynthesis : borohydride trapping of acyl-phosphate intermediates .
	manualset3
113333	5	403354	5	NULL	NULL	0	NULL	acyl-phosphate intermediates	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	MurC and MurD synthetases of peptidoglycan biosynthesis : borohydride trapping of acyl-phosphate intermediates .
	manualset3
113334	1	403355	5	NULL	NULL	0	NULL	Mural cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mural cells such as pericytes are recruited along EC tubes within these tunnel spaces to control ECM remodeling events resulting in vascular basement membrane matrix assembly , a key step in tube maturation and stabilization .
	manualset3
113335	2	403355	5	NULL	NULL	0	NULL	pericytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mural cells such as pericytes are recruited along EC tubes within these tunnel spaces to control ECM remodeling events resulting in vascular basement membrane matrix assembly , a key step in tube maturation and stabilization .
	manualset3
113336	3	403355	5	NULL	NULL	0	NULL	EC tubes 	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mural cells such as pericytes are recruited along EC tubes within these tunnel spaces to control ECM remodeling events resulting in vascular basement membrane matrix assembly , a key step in tube maturation and stabilization .
	manualset3
113337	4	403355	5	NULL	NULL	0	NULL	tunnel spaces	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mural cells such as pericytes are recruited along EC tubes within these tunnel spaces to control ECM remodeling events resulting in vascular basement membrane matrix assembly , a key step in tube maturation and stabilization .
	manualset3
113338	5	403355	5	NULL	NULL	NULL	NULL	ECM remodeling events	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mural cells such as pericytes are recruited along EC tubes within these tunnel spaces to control ECM remodeling events resulting in vascular basement membrane matrix assembly , a key step in tube maturation and stabilization .
	manualset3
113339	6	403355	5	NULL	NULL	0	NULL	vascular basement membrane matrix assembly	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mural cells such as pericytes are recruited along EC tubes within these tunnel spaces to control ECM remodeling events resulting in vascular basement membrane matrix assembly , a key step in tube maturation and stabilization .
	manualset3
113340	7	403355	5	NULL	NULL	0	NULL	key step	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mural cells such as pericytes are recruited along EC tubes within these tunnel spaces to control ECM remodeling events resulting in vascular basement membrane matrix assembly , a key step in tube maturation and stabilization .
	manualset3
113341	8	403355	5	NULL	NULL	0	NULL	tube maturation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mural cells such as pericytes are recruited along EC tubes within these tunnel spaces to control ECM remodeling events resulting in vascular basement membrane matrix assembly , a key step in tube maturation and stabilization .
	manualset3
113342	9	403355	5	NULL	NULL	0	NULL	stabilization 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mural cells such as pericytes are recruited along EC tubes within these tunnel spaces to control ECM remodeling events resulting in vascular basement membrane matrix assembly , a key step in tube maturation and stabilization .
	manualset3
113343	1	403356	5	NULL	NULL	0	NULL	Muramylpeptide shedding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Muramylpeptide shedding modulates cell sensing of Shigella flexneri .
	manualset3
113344	2	403356	5	NULL	NULL	0	NULL	cell sensing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Muramylpeptide shedding modulates cell sensing of Shigella flexneri .
	manualset3
113345	3	403356	5	NULL	NULL	0	NULL	Shigella flexneri	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Muramylpeptide shedding modulates cell sensing of Shigella flexneri .
	manualset3
113346	1	403357	5	NULL	NULL	0	NULL	Murine Flt3	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Murine Flt3 , a gene encoding a novel tyrosine kinase receptor of the PDGFR/CSF1R family .
	manualset3
113347	2	403357	5	NULL	NULL	NULL	NULL	 gene encoding a novel tyrosine kinase receptor 	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Murine Flt3 , a gene encoding a novel tyrosine kinase receptor of the PDGFR/CSF1R family .
	manualset3
113348	3	403357	5	NULL	NULL	0	NULL	PDGFR/CSF1R family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Murine Flt3 , a gene encoding a novel tyrosine kinase receptor of the PDGFR/CSF1R family .
	manualset3
113349	1	403358	5	NULL	NULL	0	NULL	Murine NK1 natural T ( NT ) cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Murine NK1 natural T ( NT ) cells are a population of alphabeta T cells that express NK cell receptors and an invariant TCR rearrangement .
	manualset3
113350	2	403358	5	NULL	NULL	0	NULL	population 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Murine NK1 natural T ( NT ) cells are a population of alphabeta T cells that express NK cell receptors and an invariant TCR rearrangement .
	manualset3
113351	3	403358	5	NULL	NULL	0	NULL	alphabeta T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Murine NK1 natural T ( NT ) cells are a population of alphabeta T cells that express NK cell receptors and an invariant TCR rearrangement .
	manualset3
113352	4	403358	5	NULL	NULL	0	NULL	NK cell receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Murine NK1 natural T ( NT ) cells are a population of alphabeta T cells that express NK cell receptors and an invariant TCR rearrangement .
	manualset3
121227	5	403358	5	NULL	NULL	0	NULL	invariant TCR rearrangement	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Murine NK1 natural T ( NT ) cells are a population of alphabeta T cells that express NK cell receptors and an invariant TCR rearrangement .
	manualset3
113353	1	403359	5	NULL	NULL	0	NULL	Murray Valley encephalitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Murray Valley encephalitis : case report and review of neuroradiological features .
	manualset3
113354	2	403359	5	NULL	NULL	0	NULL	case report 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Murray Valley encephalitis : case report and review of neuroradiological features .
	manualset3
113355	3	403359	5	NULL	NULL	0	NULL	review 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Murray Valley encephalitis : case report and review of neuroradiological features .
	manualset3
113356	4	403359	5	NULL	NULL	0	NULL	neuroradiological features	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Murray Valley encephalitis : case report and review of neuroradiological features .
	manualset3
113357	1	403360	5	NULL	NULL	0	NULL	Mus81-mediated DNA cleavage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mus81-mediated DNA cleavage resolves replication forks stalled by topoisomerase I-DNA complexes .
	manualset3
113358	2	403360	5	NULL	NULL	0	NULL	replication forks 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Mus81-mediated DNA cleavage resolves replication forks stalled by topoisomerase I-DNA complexes .
	manualset3
113359	3	403360	5	NULL	NULL	0	NULL	topoisomerase I-DNA complexes 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mus81-mediated DNA cleavage resolves replication forks stalled by topoisomerase I-DNA complexes .
	manualset3
113550	1	403361	5	NULL	NULL	0	NULL	Muscarine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscarine at a high concentration ( 10 ( -4 ) M ) only produced a 40 % increase in cAMP formation .
	manualset3
113551	2	403361	5	NULL	NULL	0	NULL	high concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscarine at a high concentration ( 10 ( -4 ) M ) only produced a 40 % increase in cAMP formation .
	manualset3
113552	3	403361	5	NULL	NULL	0	NULL	10 ( -4 ) M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscarine at a high concentration ( 10 ( -4 ) M ) only produced a 40 % increase in cAMP formation .
	manualset3
113553	4	403361	5	NULL	NULL	0	NULL	40 % increase	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscarine at a high concentration ( 10 ( -4 ) M ) only produced a 40 % increase in cAMP formation .
	manualset3
113554	5	403361	5	NULL	NULL	0	NULL	cAMP formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscarine at a high concentration ( 10 ( -4 ) M ) only produced a 40 % increase in cAMP formation .
	manualset3
113555	1	403362	5	NULL	NULL	0	NULL	Muscarinic M3 acetylcholine receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscarinic M3 acetylcholine receptors in pancreas control insulin secretion .
	manualset3
113556	2	403362	5	NULL	NULL	0	NULL	pancreas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscarinic M3 acetylcholine receptors in pancreas control insulin secretion .
	manualset3
113557	3	403362	5	NULL	NULL	0	NULL	insulin secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscarinic M3 acetylcholine receptors in pancreas control insulin secretion .
	manualset3
113558	1	403363	5	NULL	NULL	0	NULL	Muscarinic agonists	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscarinic agonists also induce and atropine potently inhibits in vitro recovery of A. caninum dauer arrest .
	manualset3
113559	2	403363	5	NULL	NULL	0	NULL	atropine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscarinic agonists also induce and atropine potently inhibits in vitro recovery of A. caninum dauer arrest .
	manualset3
113560	3	403363	5	NULL	NULL	0	NULL	 in vitro recovery	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscarinic agonists also induce and atropine potently inhibits in vitro recovery of A. caninum dauer arrest .
	manualset3
113561	4	403363	5	NULL	NULL	0	NULL	A. caninum dauer arrest	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscarinic agonists also induce and atropine potently inhibits in vitro recovery of A. caninum dauer arrest .
	manualset3
113562	1	403364	5	NULL	NULL	0	NULL	Muscle force-length properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscle and tendon force-length properties and their interactions in vivo .
	manualset3
113563	2	403364	5	NULL	NULL	0	NULL	tendon force-length properties 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscle and tendon force-length properties and their interactions in vivo .
	manualset3
113564	3	403364	5	NULL	NULL	0	NULL	interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscle and tendon force-length properties and their interactions in vivo .
	manualset3
113565	1	403365	5	NULL	NULL	0	NULL	Muscle blood flow ( MBF )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscle blood flow ( MBF ) was measured by 133Xe clearance , at rest and following exercise .
	manualset3
113566	2	403365	5	NULL	NULL	0	NULL	133Xe clearance	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscle blood flow ( MBF ) was measured by 133Xe clearance , at rest and following exercise .
	manualset3
113571	3	403365	5	NULL	NULL	0	NULL	rest	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscle blood flow ( MBF ) was measured by 133Xe clearance , at rest and following exercise .
	manualset3
113572	4	403365	5	NULL	NULL	0	NULL	exercise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscle blood flow ( MBF ) was measured by 133Xe clearance , at rest and following exercise .
	manualset3
113567	1	403366	5	NULL	NULL	0	NULL	Muscle metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscle metabolism during exercise in patients with Parkinson 's disease .
	manualset3
113568	2	403366	5	NULL	NULL	0	NULL	exercise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscle metabolism during exercise in patients with Parkinson 's disease .
	manualset3
113569	3	403366	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscle metabolism during exercise in patients with Parkinson 's disease .
	manualset3
113570	4	403366	5	NULL	NULL	0	NULL	Parkinson 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscle metabolism during exercise in patients with Parkinson 's disease .
	manualset3
113573	1	403367	5	NULL	NULL	NULL	NULL	Muscle protein kinetics	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Muscle protein kinetics were calculated during the postabsorptive state , for 2.5 h after ingestion of a meal and for 2.5 h after ingestion of an AA/CHO supplement ( EXP ) or placebo ( CON ) .
	manualset3
113574	2	403367	5	NULL	NULL	0	NULL	postabsorptive state	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscle protein kinetics were calculated during the postabsorptive state , for 2.5 h after ingestion of a meal and for 2.5 h after ingestion of an AA/CHO supplement ( EXP ) or placebo ( CON ) .
	manualset3
113575	3	403367	5	NULL	NULL	0	NULL	2.5 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscle protein kinetics were calculated during the postabsorptive state , for 2.5 h after ingestion of a meal and for 2.5 h after ingestion of an AA/CHO supplement ( EXP ) or placebo ( CON ) .
	manualset3
113576	4	403367	5	NULL	NULL	0	NULL	ingestion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscle protein kinetics were calculated during the postabsorptive state , for 2.5 h after ingestion of a meal and for 2.5 h after ingestion of an AA/CHO supplement ( EXP ) or placebo ( CON ) .
	manualset3
113577	5	403367	5	NULL	NULL	0	NULL	meal	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscle protein kinetics were calculated during the postabsorptive state , for 2.5 h after ingestion of a meal and for 2.5 h after ingestion of an AA/CHO supplement ( EXP ) or placebo ( CON ) .
	manualset3
113578	6	403367	5	NULL	NULL	0	NULL	2.5 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscle protein kinetics were calculated during the postabsorptive state , for 2.5 h after ingestion of a meal and for 2.5 h after ingestion of an AA/CHO supplement ( EXP ) or placebo ( CON ) .
	manualset3
113579	7	403367	5	NULL	NULL	0	NULL	ingestion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscle protein kinetics were calculated during the postabsorptive state , for 2.5 h after ingestion of a meal and for 2.5 h after ingestion of an AA/CHO supplement ( EXP ) or placebo ( CON ) .
	manualset3
113580	8	403367	5	NULL	NULL	0	NULL	AA/CHO supplement ( EXP )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscle protein kinetics were calculated during the postabsorptive state , for 2.5 h after ingestion of a meal and for 2.5 h after ingestion of an AA/CHO supplement ( EXP ) or placebo ( CON ) .
	manualset3
113581	9	403367	5	NULL	NULL	0	NULL	placebo ( CON )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscle protein kinetics were calculated during the postabsorptive state , for 2.5 h after ingestion of a meal and for 2.5 h after ingestion of an AA/CHO supplement ( EXP ) or placebo ( CON ) .
	manualset3
113582	1	403368	5	NULL	NULL	0	NULL	Muscular contraction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscular contraction is the nervous system 's only externally directed product , and the signaling routes which pass through the various brain components must ultimately converge on the motor areas .
	manualset3
113583	2	403368	5	NULL	NULL	0	NULL	nervous system	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscular contraction is the nervous system 's only externally directed product , and the signaling routes which pass through the various brain components must ultimately converge on the motor areas .
	manualset3
113584	3	403368	5	NULL	NULL	0	NULL	externally directed product	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscular contraction is the nervous system 's only externally directed product , and the signaling routes which pass through the various brain components must ultimately converge on the motor areas .
	manualset3
113585	4	403368	5	NULL	NULL	0	NULL	signaling routes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscular contraction is the nervous system 's only externally directed product , and the signaling routes which pass through the various brain components must ultimately converge on the motor areas .
	manualset3
113586	5	403368	5	NULL	NULL	0	NULL	brain components	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscular contraction is the nervous system 's only externally directed product , and the signaling routes which pass through the various brain components must ultimately converge on the motor areas .
	manualset3
113587	6	403368	5	NULL	NULL	0	NULL	motor areas	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscular contraction is the nervous system 's only externally directed product , and the signaling routes which pass through the various brain components must ultimately converge on the motor areas .
	manualset3
113588	1	403369	5	NULL	NULL	0	NULL	MutY	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	MutY contains three structural domains : an iron-sulfur module , a six-helix barrel module with the helix-hairpin-helix motif , and a C-terminal domain .
	manualset3
113589	2	403369	5	NULL	NULL	0	NULL	three	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	MutY contains three structural domains : an iron-sulfur module , a six-helix barrel module with the helix-hairpin-helix motif , and a C-terminal domain .
	manualset3
113590	3	403369	5	NULL	NULL	0	NULL	structural domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	MutY contains three structural domains : an iron-sulfur module , a six-helix barrel module with the helix-hairpin-helix motif , and a C-terminal domain .
	manualset3
113591	4	403369	5	NULL	NULL	0	NULL	iron-sulfur module	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	MutY contains three structural domains : an iron-sulfur module , a six-helix barrel module with the helix-hairpin-helix motif , and a C-terminal domain .
	manualset3
113592	5	403369	5	NULL	NULL	0	NULL	six-helix barrel module	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	MutY contains three structural domains : an iron-sulfur module , a six-helix barrel module with the helix-hairpin-helix motif , and a C-terminal domain .
	manualset3
113593	6	403369	5	NULL	NULL	0	NULL	helix-hairpin-helix motif 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	MutY contains three structural domains : an iron-sulfur module , a six-helix barrel module with the helix-hairpin-helix motif , and a C-terminal domain .
	manualset3
113594	7	403369	5	NULL	NULL	0	NULL	C-terminal domain 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	MutY contains three structural domains : an iron-sulfur module , a six-helix barrel module with the helix-hairpin-helix motif , and a C-terminal domain .
	manualset3
113595	1	403370	5	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A combination of A with an unreactive analog of B and a combination of B with an unreactive analog of A did not synergistically inhibit ELA proliferation .
	manualset3
113596	2	403370	5	NULL	NULL	0	NULL	A	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A combination of A with an unreactive analog of B and a combination of B with an unreactive analog of A did not synergistically inhibit ELA proliferation .
	manualset3
113597	3	403370	5	NULL	NULL	0	NULL	unreactive analog	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A combination of A with an unreactive analog of B and a combination of B with an unreactive analog of A did not synergistically inhibit ELA proliferation .
	manualset3
113598	4	403370	5	NULL	NULL	0	NULL	 B	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A combination of A with an unreactive analog of B and a combination of B with an unreactive analog of A did not synergistically inhibit ELA proliferation .
	manualset3
113599	5	403370	5	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A combination of A with an unreactive analog of B and a combination of B with an unreactive analog of A did not synergistically inhibit ELA proliferation .
	manualset3
113600	6	403370	5	NULL	NULL	0	NULL	B	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A combination of A with an unreactive analog of B and a combination of B with an unreactive analog of A did not synergistically inhibit ELA proliferation .
	manualset3
113601	7	403370	5	NULL	NULL	0	NULL	unreactive analog	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A combination of A with an unreactive analog of B and a combination of B with an unreactive analog of A did not synergistically inhibit ELA proliferation .
	manualset3
113602	8	403370	5	NULL	NULL	0	NULL	A 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A combination of A with an unreactive analog of B and a combination of B with an unreactive analog of A did not synergistically inhibit ELA proliferation .
	manualset3
113603	9	403370	5	NULL	NULL	0	NULL	ELA proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A combination of A with an unreactive analog of B and a combination of B with an unreactive analog of A did not synergistically inhibit ELA proliferation .
	manualset3
113604	1	403371	5	NULL	NULL	0	NULL	Mutant COL4A1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutant COL4A1 likely disrupts the extracellular matrix resulting in fragile vessel walls .
	manualset3
113605	2	403371	5	NULL	NULL	0	NULL	extracellular matrix	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutant COL4A1 likely disrupts the extracellular matrix resulting in fragile vessel walls .
	manualset3
113606	3	403371	5	NULL	NULL	0	NULL	fragile vessel walls	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutant COL4A1 likely disrupts the extracellular matrix resulting in fragile vessel walls .
	manualset3
113607	1	403372	5	NULL	NULL	NULL	NULL	Mutant TBEV-bc	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mutant TBEV-bc was shown to produce particles that packaged the bicistronic RNA genome and were infectious for BHK-21 cells and mice .
	manualset3
113608	2	403372	5	NULL	NULL	0	NULL	particles	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutant TBEV-bc was shown to produce particles that packaged the bicistronic RNA genome and were infectious for BHK-21 cells and mice .
	manualset3
113609	3	403372	5	NULL	NULL	0	NULL	bicistronic RNA genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutant TBEV-bc was shown to produce particles that packaged the bicistronic RNA genome and were infectious for BHK-21 cells and mice .
	manualset3
113610	4	403372	5	NULL	NULL	0	NULL	BHK-21 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutant TBEV-bc was shown to produce particles that packaged the bicistronic RNA genome and were infectious for BHK-21 cells and mice .
	manualset3
113611	5	403372	5	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutant TBEV-bc was shown to produce particles that packaged the bicistronic RNA genome and were infectious for BHK-21 cells and mice .
	manualset3
113774	1	403373	5	NULL	NULL	0	NULL	Mutant estradiol receptor alpha fragments ( H373A and H377A )	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutant estradiol receptor alpha fragments ( H373A and H377A ) lack the zinc-induced hormone release .
	manualset3
113775	2	403373	5	NULL	NULL	0	NULL	zinc-induced hormone release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutant estradiol receptor alpha fragments ( H373A and H377A ) lack the zinc-induced hormone release .
	manualset3
113776	1	403374	5	NULL	NULL	0	NULL	Mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation of other serine/threonine residues which are followed by prolines ( T79 , T89 , S117 and T155 ) together with S118 further reduced phosphorylation to around 19 % of wild-type .
	manualset3
113777	2	403374	5	NULL	NULL	0	NULL	serine/threonine residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation of other serine/threonine residues which are followed by prolines ( T79 , T89 , S117 and T155 ) together with S118 further reduced phosphorylation to around 19 % of wild-type .
	manualset3
113778	3	403374	5	NULL	NULL	0	NULL	prolines	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation of other serine/threonine residues which are followed by prolines ( T79 , T89 , S117 and T155 ) together with S118 further reduced phosphorylation to around 19 % of wild-type .
	manualset3
113779	4	403374	5	NULL	NULL	0	NULL	T79	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation of other serine/threonine residues which are followed by prolines ( T79 , T89 , S117 and T155 ) together with S118 further reduced phosphorylation to around 19 % of wild-type .
	manualset3
113780	5	403374	5	NULL	NULL	0	NULL	T89	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation of other serine/threonine residues which are followed by prolines ( T79 , T89 , S117 and T155 ) together with S118 further reduced phosphorylation to around 19 % of wild-type .
	manualset3
113781	6	403374	5	NULL	NULL	0	NULL	S117	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation of other serine/threonine residues which are followed by prolines ( T79 , T89 , S117 and T155 ) together with S118 further reduced phosphorylation to around 19 % of wild-type .
	manualset3
113782	7	403374	5	NULL	NULL	0	NULL	T155	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation of other serine/threonine residues which are followed by prolines ( T79 , T89 , S117 and T155 ) together with S118 further reduced phosphorylation to around 19 % of wild-type .
	manualset3
113783	8	403374	5	NULL	NULL	0	NULL	S118	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation of other serine/threonine residues which are followed by prolines ( T79 , T89 , S117 and T155 ) together with S118 further reduced phosphorylation to around 19 % of wild-type .
	manualset3
113784	9	403374	5	NULL	NULL	0	NULL	phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation of other serine/threonine residues which are followed by prolines ( T79 , T89 , S117 and T155 ) together with S118 further reduced phosphorylation to around 19 % of wild-type .
	manualset3
113785	10	403374	5	NULL	NULL	0	NULL	19 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation of other serine/threonine residues which are followed by prolines ( T79 , T89 , S117 and T155 ) together with S118 further reduced phosphorylation to around 19 % of wild-type .
	manualset3
113786	11	403374	5	NULL	NULL	0	NULL	wild-type	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation of other serine/threonine residues which are followed by prolines ( T79 , T89 , S117 and T155 ) together with S118 further reduced phosphorylation to around 19 % of wild-type .
	manualset3
113787	1	403375	5	NULL	NULL	0	NULL	Mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation of tyrosine 766 to phenylalanine prevented PLC-gamma activation and resulted in a reduced phosphorylation of FRS2 and reduced activation of the Ras/MEK/MAPK pathway relative to the wild-type chimeric receptor .
	manualset3
113788	2	403375	5	NULL	NULL	0	NULL	tyrosine 766	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation of tyrosine 766 to phenylalanine prevented PLC-gamma activation and resulted in a reduced phosphorylation of FRS2 and reduced activation of the Ras/MEK/MAPK pathway relative to the wild-type chimeric receptor .
	manualset3
113789	3	403375	5	NULL	NULL	0	NULL	phenylalanine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation of tyrosine 766 to phenylalanine prevented PLC-gamma activation and resulted in a reduced phosphorylation of FRS2 and reduced activation of the Ras/MEK/MAPK pathway relative to the wild-type chimeric receptor .
	manualset3
113790	4	403375	5	NULL	NULL	0	NULL	PLC-gamma activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation of tyrosine 766 to phenylalanine prevented PLC-gamma activation and resulted in a reduced phosphorylation of FRS2 and reduced activation of the Ras/MEK/MAPK pathway relative to the wild-type chimeric receptor .
	manualset3
113791	5	403375	5	NULL	NULL	0	NULL	reduced phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation of tyrosine 766 to phenylalanine prevented PLC-gamma activation and resulted in a reduced phosphorylation of FRS2 and reduced activation of the Ras/MEK/MAPK pathway relative to the wild-type chimeric receptor .
	manualset3
113792	6	403375	5	NULL	NULL	0	NULL	FRS2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation of tyrosine 766 to phenylalanine prevented PLC-gamma activation and resulted in a reduced phosphorylation of FRS2 and reduced activation of the Ras/MEK/MAPK pathway relative to the wild-type chimeric receptor .
	manualset3
113793	7	403375	5	NULL	NULL	0	NULL	reduced activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation of tyrosine 766 to phenylalanine prevented PLC-gamma activation and resulted in a reduced phosphorylation of FRS2 and reduced activation of the Ras/MEK/MAPK pathway relative to the wild-type chimeric receptor .
	manualset3
113794	8	403375	5	NULL	NULL	0	NULL	Ras/MEK/MAPK pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation of tyrosine 766 to phenylalanine prevented PLC-gamma activation and resulted in a reduced phosphorylation of FRS2 and reduced activation of the Ras/MEK/MAPK pathway relative to the wild-type chimeric receptor .
	manualset3
113795	9	403375	5	NULL	NULL	0	NULL	wild-type chimeric receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation of tyrosine 766 to phenylalanine prevented PLC-gamma activation and resulted in a reduced phosphorylation of FRS2 and reduced activation of the Ras/MEK/MAPK pathway relative to the wild-type chimeric receptor .
	manualset3
113796	1	403376	5	NULL	NULL	0	NULL	Mutational analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutational analysis of a sequence-specific ssDNA binding lupus autoantibody .
	manualset3
113797	2	403376	5	NULL	NULL	0	NULL	sequence-specific ssDNA binding lupus autoantibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutational analysis of a sequence-specific ssDNA binding lupus autoantibody .
	manualset3
113798	1	403377	5	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A combination of recent changes in the way Emergency Medical Services are reimbursed by Medicare for ambulance services and escalating costs have prompted many EMS providers to seek new ways to meet the needs of the communities they serve in a more cost-effective manner .
	manualset3
113799	2	403377	5	NULL	NULL	0	NULL	Emergency Medical Services	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A combination of recent changes in the way Emergency Medical Services are reimbursed by Medicare for ambulance services and escalating costs have prompted many EMS providers to seek new ways to meet the needs of the communities they serve in a more cost-effective manner .
	manualset3
113800	3	403377	5	NULL	NULL	0	NULL	Medicare	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A combination of recent changes in the way Emergency Medical Services are reimbursed by Medicare for ambulance services and escalating costs have prompted many EMS providers to seek new ways to meet the needs of the communities they serve in a more cost-effective manner .
	manualset3
113801	4	403377	5	NULL	NULL	0	NULL	ambulance services	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A combination of recent changes in the way Emergency Medical Services are reimbursed by Medicare for ambulance services and escalating costs have prompted many EMS providers to seek new ways to meet the needs of the communities they serve in a more cost-effective manner .
	manualset3
113802	5	403377	5	NULL	NULL	0	NULL	escalating costs	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A combination of recent changes in the way Emergency Medical Services are reimbursed by Medicare for ambulance services and escalating costs have prompted many EMS providers to seek new ways to meet the needs of the communities they serve in a more cost-effective manner .
	manualset3
113803	6	403377	5	NULL	NULL	0	NULL	EMS providers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A combination of recent changes in the way Emergency Medical Services are reimbursed by Medicare for ambulance services and escalating costs have prompted many EMS providers to seek new ways to meet the needs of the communities they serve in a more cost-effective manner .
	manualset3
113804	7	403377	5	NULL	NULL	0	NULL	new ways	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A combination of recent changes in the way Emergency Medical Services are reimbursed by Medicare for ambulance services and escalating costs have prompted many EMS providers to seek new ways to meet the needs of the communities they serve in a more cost-effective manner .
	manualset3
113805	8	403377	5	NULL	NULL	0	NULL	needs	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A combination of recent changes in the way Emergency Medical Services are reimbursed by Medicare for ambulance services and escalating costs have prompted many EMS providers to seek new ways to meet the needs of the communities they serve in a more cost-effective manner .
	manualset3
113806	9	403377	5	NULL	NULL	0	NULL	communities	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A combination of recent changes in the way Emergency Medical Services are reimbursed by Medicare for ambulance services and escalating costs have prompted many EMS providers to seek new ways to meet the needs of the communities they serve in a more cost-effective manner .
	manualset3
113807	10	403377	5	NULL	NULL	0	NULL	cost-effective manner	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A combination of recent changes in the way Emergency Medical Services are reimbursed by Medicare for ambulance services and escalating costs have prompted many EMS providers to seek new ways to meet the needs of the communities they serve in a more cost-effective manner .
	manualset3
116803	11	403377	5	NULL	NULL	0	NULL	recent changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A combination of recent changes in the way Emergency Medical Services are reimbursed by Medicare for ambulance services and escalating costs have prompted many EMS providers to seek new ways to meet the needs of the communities they serve in a more cost-effective manner .
	manualset3
113808	1	403378	5	NULL	NULL	0	NULL	Mutational analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutational analysis of the hMSH2 gene reveals a three base pair deletion in a family predisposed to colorectal cancer development .
	manualset3
113809	2	403378	5	NULL	NULL	0	NULL	hMSH2 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutational analysis of the hMSH2 gene reveals a three base pair deletion in a family predisposed to colorectal cancer development .
	manualset3
113810	3	403378	5	NULL	NULL	0	NULL	three base pair deletion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutational analysis of the hMSH2 gene reveals a three base pair deletion in a family predisposed to colorectal cancer development .
	manualset3
113811	4	403378	5	NULL	NULL	0	NULL	family	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutational analysis of the hMSH2 gene reveals a three base pair deletion in a family predisposed to colorectal cancer development .
	manualset3
113812	5	403378	5	NULL	NULL	0	NULL	colorectal cancer development 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutational analysis of the hMSH2 gene reveals a three base pair deletion in a family predisposed to colorectal cancer development .
	manualset3
113813	1	403379	5	NULL	NULL	0	NULL	Mutational and expression analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutational and expression analysis in primary CLL samples failed to demonstrate any specific mutations in DLEU7 , but no DLEU7 expression could be detected in CLL cells .
	manualset3
113814	2	403379	5	NULL	NULL	0	NULL	primary CLL samples	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutational and expression analysis in primary CLL samples failed to demonstrate any specific mutations in DLEU7 , but no DLEU7 expression could be detected in CLL cells .
	manualset3
113815	3	403379	5	NULL	NULL	0	NULL	specific mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutational and expression analysis in primary CLL samples failed to demonstrate any specific mutations in DLEU7 , but no DLEU7 expression could be detected in CLL cells .
	manualset3
113816	4	403379	5	NULL	NULL	0	NULL	DLEU7	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutational and expression analysis in primary CLL samples failed to demonstrate any specific mutations in DLEU7 , but no DLEU7 expression could be detected in CLL cells .
	manualset3
113817	5	403379	5	NULL	NULL	0	NULL	DLEU7 expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutational and expression analysis in primary CLL samples failed to demonstrate any specific mutations in DLEU7 , but no DLEU7 expression could be detected in CLL cells .
	manualset3
113818	6	403379	5	NULL	NULL	0	NULL	CLL cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutational and expression analysis in primary CLL samples failed to demonstrate any specific mutations in DLEU7 , but no DLEU7 expression could be detected in CLL cells .
	manualset3
113819	1	403380	5	NULL	NULL	0	NULL	Mutations Y181C	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations Y181C , Y181I , and Y188L led to reduced sensitivity , albeit of varying extents , to all HIV-1-specific RT inhibitors .
	manualset3
113820	2	403380	5	NULL	NULL	0	NULL	Mutations Y181I	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations Y181C , Y181I , and Y188L led to reduced sensitivity , albeit of varying extents , to all HIV-1-specific RT inhibitors .
	manualset3
113821	3	403380	5	NULL	NULL	0	NULL	Mutations Y188L	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations Y181C , Y181I , and Y188L led to reduced sensitivity , albeit of varying extents , to all HIV-1-specific RT inhibitors .
	manualset3
113822	4	403380	5	NULL	NULL	0	NULL	reduced sensitivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations Y181C , Y181I , and Y188L led to reduced sensitivity , albeit of varying extents , to all HIV-1-specific RT inhibitors .
	manualset3
113823	5	403380	5	NULL	NULL	0	NULL	HIV-1-specific RT inhibitors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations Y181C , Y181I , and Y188L led to reduced sensitivity , albeit of varying extents , to all HIV-1-specific RT inhibitors .
	manualset3
113824	1	403381	5	NULL	NULL	0	NULL	Mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations at the c-kit locus resulted in deficiency of MMC and CTMC in both mice and rats .
	manualset3
113825	2	403381	5	NULL	NULL	0	NULL	c-kit locus 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations at the c-kit locus resulted in deficiency of MMC and CTMC in both mice and rats .
	manualset3
113873	3	403381	5	NULL	NULL	0	NULL	deficiency 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations at the c-kit locus resulted in deficiency of MMC and CTMC in both mice and rats .
	manualset3
113882	4	403381	5	NULL	NULL	0	NULL	MMC 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations at the c-kit locus resulted in deficiency of MMC and CTMC in both mice and rats .
	manualset3
113883	5	403381	5	NULL	NULL	0	NULL	CTMC 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations at the c-kit locus resulted in deficiency of MMC and CTMC in both mice and rats .
	manualset3
113884	6	403381	5	NULL	NULL	0	NULL	mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations at the c-kit locus resulted in deficiency of MMC and CTMC in both mice and rats .
	manualset3
113885	7	403381	5	NULL	NULL	0	NULL	rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations at the c-kit locus resulted in deficiency of MMC and CTMC in both mice and rats .
	manualset3
113886	1	403382	5	NULL	NULL	0	NULL	Mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in NNT encoding nicotinamide nucleotide transhydrogenase cause familial glucocorticoid deficiency .
	manualset3
113887	2	403382	5	NULL	NULL	0	NULL	NNT encoding nicotinamide nucleotide transhydrogenase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in NNT encoding nicotinamide nucleotide transhydrogenase cause familial glucocorticoid deficiency .
	manualset3
113888	3	403382	5	NULL	NULL	0	NULL	familial glucocorticoid deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in NNT encoding nicotinamide nucleotide transhydrogenase cause familial glucocorticoid deficiency .
	manualset3
113889	1	403383	5	NULL	NULL	0	NULL	Mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in one of the duplicated survival of motor neuron ( SMN ) genes lead to the progressive loss of motor neurons and subsequent development of spinal muscular atrophy ( SMA ) , a common , and usually fatal , hereditary disease .
	manualset3
113890	2	403383	5	NULL	NULL	0	NULL	survival of motor neuron ( SMN ) genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in one of the duplicated survival of motor neuron ( SMN ) genes lead to the progressive loss of motor neurons and subsequent development of spinal muscular atrophy ( SMA ) , a common , and usually fatal , hereditary disease .
	manualset3
113891	3	403383	5	NULL	NULL	0	NULL	progressive loss	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in one of the duplicated survival of motor neuron ( SMN ) genes lead to the progressive loss of motor neurons and subsequent development of spinal muscular atrophy ( SMA ) , a common , and usually fatal , hereditary disease .
	manualset3
113892	4	403383	5	NULL	NULL	0	NULL	motor neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in one of the duplicated survival of motor neuron ( SMN ) genes lead to the progressive loss of motor neurons and subsequent development of spinal muscular atrophy ( SMA ) , a common , and usually fatal , hereditary disease .
	manualset3
113893	5	403383	5	NULL	NULL	NULL	NULL	subsequent development	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mutations in one of the duplicated survival of motor neuron ( SMN ) genes lead to the progressive loss of motor neurons and subsequent development of spinal muscular atrophy ( SMA ) , a common , and usually fatal , hereditary disease .
	manualset3
113894	6	403383	5	NULL	NULL	0	NULL	spinal muscular atrophy ( SMA )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in one of the duplicated survival of motor neuron ( SMN ) genes lead to the progressive loss of motor neurons and subsequent development of spinal muscular atrophy ( SMA ) , a common , and usually fatal , hereditary disease .
	manualset3
113895	7	403383	5	NULL	NULL	0	NULL	hereditary disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in one of the duplicated survival of motor neuron ( SMN ) genes lead to the progressive loss of motor neurons and subsequent development of spinal muscular atrophy ( SMA ) , a common , and usually fatal , hereditary disease .
	manualset3
113896	1	403384	5	NULL	NULL	0	NULL	Mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in purR ( s ) or in the purD operator accumulated when the mutant strain was placed on a minimal lactose plate supplemented with 10 microg/ml of adenine during prolonged incubation .
	manualset3
113897	2	403384	5	NULL	NULL	0	NULL	purR ( s )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in purR ( s ) or in the purD operator accumulated when the mutant strain was placed on a minimal lactose plate supplemented with 10 microg/ml of adenine during prolonged incubation .
	manualset3
113898	3	403384	5	NULL	NULL	0	NULL	purD operator 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in purR ( s ) or in the purD operator accumulated when the mutant strain was placed on a minimal lactose plate supplemented with 10 microg/ml of adenine during prolonged incubation .
	manualset3
113899	4	403384	5	NULL	NULL	0	NULL	mutant strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in purR ( s ) or in the purD operator accumulated when the mutant strain was placed on a minimal lactose plate supplemented with 10 microg/ml of adenine during prolonged incubation .
	manualset3
113900	5	403384	5	NULL	NULL	0	NULL	minimal lactose plate	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in purR ( s ) or in the purD operator accumulated when the mutant strain was placed on a minimal lactose plate supplemented with 10 microg/ml of adenine during prolonged incubation .
	manualset3
113901	6	403384	5	NULL	NULL	0	NULL	10 microg/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in purR ( s ) or in the purD operator accumulated when the mutant strain was placed on a minimal lactose plate supplemented with 10 microg/ml of adenine during prolonged incubation .
	manualset3
113902	7	403384	5	NULL	NULL	0	NULL	adenine 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in purR ( s ) or in the purD operator accumulated when the mutant strain was placed on a minimal lactose plate supplemented with 10 microg/ml of adenine during prolonged incubation .
	manualset3
113903	8	403384	5	NULL	NULL	0	NULL	prolonged incubation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in purR ( s ) or in the purD operator accumulated when the mutant strain was placed on a minimal lactose plate supplemented with 10 microg/ml of adenine during prolonged incubation .
	manualset3
113904	1	403385	5	NULL	NULL	0	NULL	Mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the gene encoding the CYP2C-19 enzyme for PPI metabolism have been shown to enhance the chance for a cure in a H. pylori-positive patients using a two-week dual-therapy regimen involving omeprazole and amoxicillin .
	manualset3
113905	2	403385	5	NULL	NULL	0	NULL	gene encoding the CYP2C-19 enzyme	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the gene encoding the CYP2C-19 enzyme for PPI metabolism have been shown to enhance the chance for a cure in a H. pylori-positive patients using a two-week dual-therapy regimen involving omeprazole and amoxicillin .
	manualset3
113978	3	403385	5	NULL	NULL	0	NULL	PPI metabolism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the gene encoding the CYP2C-19 enzyme for PPI metabolism have been shown to enhance the chance for a cure in a H. pylori-positive patients using a two-week dual-therapy regimen involving omeprazole and amoxicillin .
	manualset3
113980	4	403385	5	NULL	NULL	0	NULL	cure 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the gene encoding the CYP2C-19 enzyme for PPI metabolism have been shown to enhance the chance for a cure in a H. pylori-positive patients using a two-week dual-therapy regimen involving omeprazole and amoxicillin .
	manualset3
113982	5	403385	5	NULL	NULL	0	NULL	H. pylori-positive patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the gene encoding the CYP2C-19 enzyme for PPI metabolism have been shown to enhance the chance for a cure in a H. pylori-positive patients using a two-week dual-therapy regimen involving omeprazole and amoxicillin .
	manualset3
113984	6	403385	5	NULL	NULL	0	NULL	two-week dual-therapy regimen	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the gene encoding the CYP2C-19 enzyme for PPI metabolism have been shown to enhance the chance for a cure in a H. pylori-positive patients using a two-week dual-therapy regimen involving omeprazole and amoxicillin .
	manualset3
113986	7	403385	5	NULL	NULL	0	NULL	omeprazole 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the gene encoding the CYP2C-19 enzyme for PPI metabolism have been shown to enhance the chance for a cure in a H. pylori-positive patients using a two-week dual-therapy regimen involving omeprazole and amoxicillin .
	manualset3
113987	8	403385	5	NULL	NULL	0	NULL	amoxicillin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the gene encoding the CYP2C-19 enzyme for PPI metabolism have been shown to enhance the chance for a cure in a H. pylori-positive patients using a two-week dual-therapy regimen involving omeprazole and amoxicillin .
	manualset3
113997	1	403386	5	NULL	NULL	0	NULL	Mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the mitochondrial kinase PINK1 and the cytosolic E3 ligase Parkin can cause Parkinson 's disease .
	manualset3
113998	2	403386	5	NULL	NULL	0	NULL	mitochondrial kinase PINK1	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the mitochondrial kinase PINK1 and the cytosolic E3 ligase Parkin can cause Parkinson 's disease .
	manualset3
113999	3	403386	5	NULL	NULL	0	NULL	cytosolic E3 ligase Parkin	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the mitochondrial kinase PINK1 and the cytosolic E3 ligase Parkin can cause Parkinson 's disease .
	manualset3
114000	4	403386	5	NULL	NULL	0	NULL	Parkinson 's disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the mitochondrial kinase PINK1 and the cytosolic E3 ligase Parkin can cause Parkinson 's disease .
	manualset3
114001	1	403387	5	NULL	NULL	0	NULL	Mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations of the cyclic nucleotide binding domain ( CNBD ) may disrupt human ether-a-go-go-related gene ( hERG ) K ( + ) channel function and lead to hereditary long QT syndrome ( LQTS ) .
	manualset3
114002	2	403387	5	NULL	NULL	0	NULL	cyclic nucleotide binding domain ( CNBD ) 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations of the cyclic nucleotide binding domain ( CNBD ) may disrupt human ether-a-go-go-related gene ( hERG ) K ( + ) channel function and lead to hereditary long QT syndrome ( LQTS ) .
	manualset3
114003	3	403387	5	NULL	NULL	0	NULL	human ether-a-go-go-related gene ( hERG )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations of the cyclic nucleotide binding domain ( CNBD ) may disrupt human ether-a-go-go-related gene ( hERG ) K ( + ) channel function and lead to hereditary long QT syndrome ( LQTS ) .
	manualset3
114004	4	403387	5	NULL	NULL	0	NULL	K ( + ) channel function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations of the cyclic nucleotide binding domain ( CNBD ) may disrupt human ether-a-go-go-related gene ( hERG ) K ( + ) channel function and lead to hereditary long QT syndrome ( LQTS ) .
	manualset3
114005	5	403387	5	NULL	NULL	0	NULL	hereditary long QT syndrome ( LQTS ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations of the cyclic nucleotide binding domain ( CNBD ) may disrupt human ether-a-go-go-related gene ( hERG ) K ( + ) channel function and lead to hereditary long QT syndrome ( LQTS ) .
	manualset3
114006	1	403388	5	NULL	NULL	0	NULL	Mycelium 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycelium of Rhizopus nigricans when stained with certain acid and basic dyes and washed with buffer mixtures of 0.1 M phosphoric acid and sodium hydroxide responded much like an amphoteric colloid with an isoelectric point near pH 5.0 .
	manualset3
114008	2	403388	5	NULL	NULL	0	NULL	Rhizopus nigricans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycelium of Rhizopus nigricans when stained with certain acid and basic dyes and washed with buffer mixtures of 0.1 M phosphoric acid and sodium hydroxide responded much like an amphoteric colloid with an isoelectric point near pH 5.0 .
	manualset3
114010	3	403388	5	NULL	NULL	0	NULL	acid dyes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycelium of Rhizopus nigricans when stained with certain acid and basic dyes and washed with buffer mixtures of 0.1 M phosphoric acid and sodium hydroxide responded much like an amphoteric colloid with an isoelectric point near pH 5.0 .
	manualset3
114011	4	403388	5	NULL	NULL	0	NULL	basic dyes 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycelium of Rhizopus nigricans when stained with certain acid and basic dyes and washed with buffer mixtures of 0.1 M phosphoric acid and sodium hydroxide responded much like an amphoteric colloid with an isoelectric point near pH 5.0 .
	manualset3
114012	5	403388	5	NULL	NULL	0	NULL	buffer mixtures	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycelium of Rhizopus nigricans when stained with certain acid and basic dyes and washed with buffer mixtures of 0.1 M phosphoric acid and sodium hydroxide responded much like an amphoteric colloid with an isoelectric point near pH 5.0 .
	manualset3
114017	6	403388	5	NULL	NULL	0	NULL	0.1 M 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycelium of Rhizopus nigricans when stained with certain acid and basic dyes and washed with buffer mixtures of 0.1 M phosphoric acid and sodium hydroxide responded much like an amphoteric colloid with an isoelectric point near pH 5.0 .
	manualset3
114019	7	403388	5	NULL	NULL	0	NULL	phosphoric acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycelium of Rhizopus nigricans when stained with certain acid and basic dyes and washed with buffer mixtures of 0.1 M phosphoric acid and sodium hydroxide responded much like an amphoteric colloid with an isoelectric point near pH 5.0 .
	manualset3
114022	8	403388	5	NULL	NULL	0	NULL	sodium hydroxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycelium of Rhizopus nigricans when stained with certain acid and basic dyes and washed with buffer mixtures of 0.1 M phosphoric acid and sodium hydroxide responded much like an amphoteric colloid with an isoelectric point near pH 5.0 .
	manualset3
114024	9	403388	5	NULL	NULL	0	NULL	amphoteric colloid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycelium of Rhizopus nigricans when stained with certain acid and basic dyes and washed with buffer mixtures of 0.1 M phosphoric acid and sodium hydroxide responded much like an amphoteric colloid with an isoelectric point near pH 5.0 .
	manualset3
114026	10	403388	5	NULL	NULL	0	NULL	isoelectric point 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycelium of Rhizopus nigricans when stained with certain acid and basic dyes and washed with buffer mixtures of 0.1 M phosphoric acid and sodium hydroxide responded much like an amphoteric colloid with an isoelectric point near pH 5.0 .
	manualset3
114028	11	403388	5	NULL	NULL	0	NULL	pH 5.0	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycelium of Rhizopus nigricans when stained with certain acid and basic dyes and washed with buffer mixtures of 0.1 M phosphoric acid and sodium hydroxide responded much like an amphoteric colloid with an isoelectric point near pH 5.0 .
	manualset3
114032	1	403389	5	NULL	NULL	0	NULL	Mycetoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycetoma : infection with tumefaction , draining sinuses , and `` grains '' .
	manualset3
114033	2	403389	5	NULL	NULL	0	NULL	infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycetoma : infection with tumefaction , draining sinuses , and `` grains '' .
	manualset3
114034	3	403389	5	NULL	NULL	0	NULL	tumefaction 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycetoma : infection with tumefaction , draining sinuses , and `` grains '' .
	manualset3
114038	4	403389	5	NULL	NULL	0	NULL	draining sinuses	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycetoma : infection with tumefaction , draining sinuses , and `` grains '' .
	manualset3
114045	5	403389	5	NULL	NULL	0	NULL	grains 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycetoma : infection with tumefaction , draining sinuses , and `` grains '' .
	manualset3
114046	1	403390	5	NULL	NULL	0	NULL	Mycobacterial infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycobacterial infections in AIDS : an overview of epidemiology , clinical manifestations , therapy and prophylaxis .
	manualset3
114047	2	403390	5	NULL	NULL	0	NULL	AIDS 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycobacterial infections in AIDS : an overview of epidemiology , clinical manifestations , therapy and prophylaxis .
	manualset3
114049	3	403390	5	NULL	NULL	0	NULL	overview 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycobacterial infections in AIDS : an overview of epidemiology , clinical manifestations , therapy and prophylaxis .
	manualset3
114050	4	403390	5	NULL	NULL	0	NULL	epidemiology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycobacterial infections in AIDS : an overview of epidemiology , clinical manifestations , therapy and prophylaxis .
	manualset3
114054	5	403390	5	NULL	NULL	0	NULL	clinical manifestations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycobacterial infections in AIDS : an overview of epidemiology , clinical manifestations , therapy and prophylaxis .
	manualset3
114056	6	403390	5	NULL	NULL	0	NULL	therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycobacterial infections in AIDS : an overview of epidemiology , clinical manifestations , therapy and prophylaxis .
	manualset3
114057	7	403390	5	NULL	NULL	0	NULL	prophylaxis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycobacterial infections in AIDS : an overview of epidemiology , clinical manifestations , therapy and prophylaxis .
	manualset3
114058	1	403391	5	NULL	NULL	0	NULL	Mycobacteriophage L5	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycobacteriophage L5 is a temperate phage that forms lysogens in Mycobacterium smegmatis .
	manualset3
114059	2	403391	5	NULL	NULL	0	NULL	temperate phage	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycobacteriophage L5 is a temperate phage that forms lysogens in Mycobacterium smegmatis .
	manualset3
114234	3	403391	5	NULL	NULL	0	NULL	lysogens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycobacteriophage L5 is a temperate phage that forms lysogens in Mycobacterium smegmatis .
	manualset3
114235	4	403391	5	NULL	NULL	0	NULL	Mycobacterium smegmatis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycobacteriophage L5 is a temperate phage that forms lysogens in Mycobacterium smegmatis .
	manualset3
114239	1	403392	5	NULL	NULL	0	NULL	Mycophenolic acid ( MPA )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycophenolic acid ( MPA ) , an inhibitor of IMP dehydrogenase , inhibits reovirus replication and viral RNA and protein production .
	manualset3
114240	2	403392	5	NULL	NULL	0	NULL	inhibitor	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycophenolic acid ( MPA ) , an inhibitor of IMP dehydrogenase , inhibits reovirus replication and viral RNA and protein production .
	manualset3
114242	3	403392	5	NULL	NULL	0	NULL	IMP dehydrogenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycophenolic acid ( MPA ) , an inhibitor of IMP dehydrogenase , inhibits reovirus replication and viral RNA and protein production .
	manualset3
114244	4	403392	5	NULL	NULL	0	NULL	reovirus replication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycophenolic acid ( MPA ) , an inhibitor of IMP dehydrogenase , inhibits reovirus replication and viral RNA and protein production .
	manualset3
114246	5	403392	5	NULL	NULL	0	NULL	viral RNA production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycophenolic acid ( MPA ) , an inhibitor of IMP dehydrogenase , inhibits reovirus replication and viral RNA and protein production .
	manualset3
114247	6	403392	5	NULL	NULL	0	NULL	protein production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycophenolic acid ( MPA ) , an inhibitor of IMP dehydrogenase , inhibits reovirus replication and viral RNA and protein production .
	manualset3
114252	1	403393	5	NULL	NULL	0	NULL	Mycophenolic acid pharmacokinetics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycophenolic acid pharmacokinetics during maintenance immunosuppression in African American and Caucasian renal transplant recipients .
	manualset3
114254	2	403393	5	NULL	NULL	0	NULL	maintenance immunosuppression	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycophenolic acid pharmacokinetics during maintenance immunosuppression in African American and Caucasian renal transplant recipients .
	manualset3
114256	3	403393	5	NULL	NULL	0	NULL	African American renal transplant recipients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycophenolic acid pharmacokinetics during maintenance immunosuppression in African American and Caucasian renal transplant recipients .
	manualset3
114259	4	403393	5	NULL	NULL	0	NULL	Caucasian renal transplant recipients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycophenolic acid pharmacokinetics during maintenance immunosuppression in African American and Caucasian renal transplant recipients .
	manualset3
114262	1	403394	5	NULL	NULL	0	NULL	Mycosis fungoides	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycosis fungoides is the most common form of cutaneous T-cell lymphomas .
	manualset3
114263	2	403394	5	NULL	NULL	0	NULL	cutaneous T-cell lymphomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycosis fungoides is the most common form of cutaneous T-cell lymphomas .
	manualset3
114264	1	403395	5	NULL	NULL	0	NULL	immunocytochemical study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A combined immunocytochemical and retrograde tracing study of noradrenergic connections between the caudal medulla and bed nuclei of the stria terminalis .
	manualset3
114265	2	403395	5	NULL	NULL	0	NULL	retrograde tracing study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A combined immunocytochemical and retrograde tracing study of noradrenergic connections between the caudal medulla and bed nuclei of the stria terminalis .
	manualset3
114266	3	403395	5	NULL	NULL	0	NULL	noradrenergic connections 	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A combined immunocytochemical and retrograde tracing study of noradrenergic connections between the caudal medulla and bed nuclei of the stria terminalis .
	manualset3
114267	4	403395	5	NULL	NULL	0	NULL	caudal medulla	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A combined immunocytochemical and retrograde tracing study of noradrenergic connections between the caudal medulla and bed nuclei of the stria terminalis .
	manualset3
114268	5	403395	5	NULL	NULL	0	NULL	bed nuclei	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A combined immunocytochemical and retrograde tracing study of noradrenergic connections between the caudal medulla and bed nuclei of the stria terminalis .
	manualset3
114269	6	403395	5	NULL	NULL	0	NULL	stria terminalis	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A combined immunocytochemical and retrograde tracing study of noradrenergic connections between the caudal medulla and bed nuclei of the stria terminalis .
	manualset3
114270	1	403396	5	NULL	NULL	0	NULL	Myelin breakdown	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Myelin breakdown in the posterior funiculus of the kitten after dorsal rhizotomy .
	manualset3
114271	2	403396	5	NULL	NULL	0	NULL	posterior funiculus	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Myelin breakdown in the posterior funiculus of the kitten after dorsal rhizotomy .
	manualset3
114272	3	403396	5	NULL	NULL	0	NULL	kitten	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Myelin breakdown in the posterior funiculus of the kitten after dorsal rhizotomy .
	manualset3
114273	4	403396	5	NULL	NULL	0	NULL	dorsal rhizotomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Myelin breakdown in the posterior funiculus of the kitten after dorsal rhizotomy .
	manualset3
114274	1	403397	5	NULL	NULL	0	NULL	Myeloarchitecture	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Myelo - and cytoarchitecture of the granular frontal cortex and surrounding regions in the strepsirhine primate Galago and the anthropoid primate Macaca .
	manualset3
114275	2	403397	5	NULL	NULL	0	NULL	cytoarchitecture	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Myelo - and cytoarchitecture of the granular frontal cortex and surrounding regions in the strepsirhine primate Galago and the anthropoid primate Macaca .
	manualset3
114276	3	403397	5	NULL	NULL	0	NULL	granular frontal cortex	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Myelo - and cytoarchitecture of the granular frontal cortex and surrounding regions in the strepsirhine primate Galago and the anthropoid primate Macaca .
	manualset3
114277	4	403397	5	NULL	NULL	0	NULL	surrounding regions	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Myelo - and cytoarchitecture of the granular frontal cortex and surrounding regions in the strepsirhine primate Galago and the anthropoid primate Macaca .
	manualset3
114278	5	403397	5	NULL	NULL	0	NULL	strepsirhine primate Galago	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Myelo - and cytoarchitecture of the granular frontal cortex and surrounding regions in the strepsirhine primate Galago and the anthropoid primate Macaca .
	manualset3
114279	6	403397	5	NULL	NULL	0	NULL	anthropoid primate Macaca	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Myelo - and cytoarchitecture of the granular frontal cortex and surrounding regions in the strepsirhine primate Galago and the anthropoid primate Macaca .
	manualset3
114280	1	403398	5	NULL	NULL	0	NULL	Myelography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Myelography and cerebrospinal fluid analysis revealed severe hydromyelia and myelitis , respectively .
	manualset3
114281	2	403398	5	NULL	NULL	0	NULL	cerebrospinal fluid analysis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Myelography and cerebrospinal fluid analysis revealed severe hydromyelia and myelitis , respectively .
	manualset3
114282	3	403398	5	NULL	NULL	0	NULL	severe hydromyelia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Myelography and cerebrospinal fluid analysis revealed severe hydromyelia and myelitis , respectively .
	manualset3
114283	4	403398	5	NULL	NULL	0	NULL	myelitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Myelography and cerebrospinal fluid analysis revealed severe hydromyelia and myelitis , respectively .
	manualset3
114284	1	403399	5	NULL	NULL	0	NULL	Myeloma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Myeloma cells from seven MM cell lines with mutated or w.t. p53 and varying expression of bcl-2 were used .
	manualset3
114285	2	403399	5	NULL	NULL	0	NULL	seven	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Myeloma cells from seven MM cell lines with mutated or w.t. p53 and varying expression of bcl-2 were used .
	manualset3
114286	3	403399	5	NULL	NULL	0	NULL	MM cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Myeloma cells from seven MM cell lines with mutated or w.t. p53 and varying expression of bcl-2 were used .
	manualset3
114287	4	403399	5	NULL	NULL	0	NULL	w.t. p53	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Myeloma cells from seven MM cell lines with mutated or w.t. p53 and varying expression of bcl-2 were used .
	manualset3
114288	5	403399	5	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Myeloma cells from seven MM cell lines with mutated or w.t. p53 and varying expression of bcl-2 were used .
	manualset3
114289	6	403399	5	NULL	NULL	0	NULL	bcl-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Myeloma cells from seven MM cell lines with mutated or w.t. p53 and varying expression of bcl-2 were used .
	manualset3
114290	1	403400	5	NULL	NULL	0	NULL	MyoD	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	MyoD , a master regulator of myogenesis , exhibits a circadian rhythm in its mRNA and protein levels , suggesting a possible role in the daily maintenance of muscle phenotype and function .
	manualset3
114291	2	403400	5	NULL	NULL	0	NULL	master regulator	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	MyoD , a master regulator of myogenesis , exhibits a circadian rhythm in its mRNA and protein levels , suggesting a possible role in the daily maintenance of muscle phenotype and function .
	manualset3
114292	3	403400	5	NULL	NULL	0	NULL	myogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MyoD , a master regulator of myogenesis , exhibits a circadian rhythm in its mRNA and protein levels , suggesting a possible role in the daily maintenance of muscle phenotype and function .
	manualset3
114293	4	403400	5	NULL	NULL	0	NULL	circadian rhythm	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MyoD , a master regulator of myogenesis , exhibits a circadian rhythm in its mRNA and protein levels , suggesting a possible role in the daily maintenance of muscle phenotype and function .
	manualset3
114294	5	403400	5	NULL	NULL	NULL	NULL	mRNA levels	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	MyoD , a master regulator of myogenesis , exhibits a circadian rhythm in its mRNA and protein levels , suggesting a possible role in the daily maintenance of muscle phenotype and function .
	manualset3
114295	6	403400	5	NULL	NULL	0	NULL	protein levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	MyoD , a master regulator of myogenesis , exhibits a circadian rhythm in its mRNA and protein levels , suggesting a possible role in the daily maintenance of muscle phenotype and function .
	manualset3
114296	7	403400	5	NULL	NULL	0	NULL	possible role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MyoD , a master regulator of myogenesis , exhibits a circadian rhythm in its mRNA and protein levels , suggesting a possible role in the daily maintenance of muscle phenotype and function .
	manualset3
114297	8	403400	5	NULL	NULL	0	NULL	daily maintenance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MyoD , a master regulator of myogenesis , exhibits a circadian rhythm in its mRNA and protein levels , suggesting a possible role in the daily maintenance of muscle phenotype and function .
	manualset3
114298	9	403400	5	NULL	NULL	0	NULL	muscle phenotype	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MyoD , a master regulator of myogenesis , exhibits a circadian rhythm in its mRNA and protein levels , suggesting a possible role in the daily maintenance of muscle phenotype and function .
	manualset3
114299	10	403400	5	NULL	NULL	0	NULL	function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MyoD , a master regulator of myogenesis , exhibits a circadian rhythm in its mRNA and protein levels , suggesting a possible role in the daily maintenance of muscle phenotype and function .
	manualset3
114300	1	403401	5	NULL	NULL	0	NULL	Myocardial concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Myocardial concentration of norepinephrine and cyclic AMP in ventricular fibrillation during acute myocardial ischemia .
	manualset3
114301	2	403401	5	NULL	NULL	0	NULL	norepinephrine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Myocardial concentration of norepinephrine and cyclic AMP in ventricular fibrillation during acute myocardial ischemia .
	manualset3
114302	3	403401	5	NULL	NULL	0	NULL	cyclic AMP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Myocardial concentration of norepinephrine and cyclic AMP in ventricular fibrillation during acute myocardial ischemia .
	manualset3
114303	4	403401	5	NULL	NULL	0	NULL	ventricular fibrillation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Myocardial concentration of norepinephrine and cyclic AMP in ventricular fibrillation during acute myocardial ischemia .
	manualset3
114304	5	403401	5	NULL	NULL	0	NULL	acute myocardial ischemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Myocardial concentration of norepinephrine and cyclic AMP in ventricular fibrillation during acute myocardial ischemia .
	manualset3
114305	1	403402	5	NULL	NULL	0	NULL	Myocardial injury 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Myocardial injury was induced by administering graded doses of isoproterenol ( ISO ) for 15 days .
	manualset3
114306	2	403402	5	NULL	NULL	0	NULL	graded doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Myocardial injury was induced by administering graded doses of isoproterenol ( ISO ) for 15 days .
	manualset3
114307	3	403402	5	NULL	NULL	0	NULL	isoproterenol ( ISO )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Myocardial injury was induced by administering graded doses of isoproterenol ( ISO ) for 15 days .
	manualset3
114308	4	403402	5	NULL	NULL	0	NULL	15 days	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Myocardial injury was induced by administering graded doses of isoproterenol ( ISO ) for 15 days .
	manualset3
114309	1	403403	5	NULL	NULL	0	NULL	Myocardial preservation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Myocardial preservation with nifedipine : a comparative study at normothermia .
	manualset3
114310	2	403403	5	NULL	NULL	0	NULL	nifedipine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Myocardial preservation with nifedipine : a comparative study at normothermia .
	manualset3
114311	3	403403	5	NULL	NULL	0	NULL	comparative study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Myocardial preservation with nifedipine : a comparative study at normothermia .
	manualset3
114312	4	403403	5	NULL	NULL	0	NULL	normothermia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Myocardial preservation with nifedipine : a comparative study at normothermia .
	manualset3
114313	1	403404	5	NULL	NULL	0	NULL	Myofilament	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Myofilament Ca-sensitivity and SR function were unaffected by .
	manualset3
114314	2	403404	5	NULL	NULL	0	NULL	Ca-sensitivity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Myofilament Ca-sensitivity and SR function were unaffected by .
	manualset3
114315	3	403404	5	NULL	NULL	NULL	NULL	SR function	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Myofilament Ca-sensitivity and SR function were unaffected by .
	manualset3
114316	1	403405	5	NULL	NULL	0	NULL	Myosin II inhibition 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Myosin II inhibition caused a loss of peripheral F-actin bundles and a submembranous extension of cortical microtubules .
	manualset3
114317	2	403405	5	NULL	NULL	0	NULL	loss 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Myosin II inhibition caused a loss of peripheral F-actin bundles and a submembranous extension of cortical microtubules .
	manualset3
114318	3	403405	5	NULL	NULL	0	NULL	peripheral F-actin bundles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Myosin II inhibition caused a loss of peripheral F-actin bundles and a submembranous extension of cortical microtubules .
	manualset3
114319	4	403405	5	NULL	NULL	0	NULL	submembranous extension 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Myosin II inhibition caused a loss of peripheral F-actin bundles and a submembranous extension of cortical microtubules .
	manualset3
114320	5	403405	5	NULL	NULL	0	NULL	cortical microtubules 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Myosin II inhibition caused a loss of peripheral F-actin bundles and a submembranous extension of cortical microtubules .
	manualset3
114321	1	403406	5	NULL	NULL	0	NULL	Myosin light chain phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Myosin light chain phosphorylation and pulmonary endothelial cell hyperpermeability in burns .
	manualset3
114322	2	403406	5	NULL	NULL	0	NULL	pulmonary endothelial cell hyperpermeability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Myosin light chain phosphorylation and pulmonary endothelial cell hyperpermeability in burns .
	manualset3
114323	3	403406	5	NULL	NULL	0	NULL	burns 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Myosin light chain phosphorylation and pulmonary endothelial cell hyperpermeability in burns .
	manualset3
114324	1	403407	5	NULL	NULL	0	NULL	Myostatin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Myostatin regulates preadipocyte differentiation and lipid metabolism of adipocyte via ERK1/2 .
	manualset3
114325	2	403407	5	NULL	NULL	0	NULL	preadipocyte differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Myostatin regulates preadipocyte differentiation and lipid metabolism of adipocyte via ERK1/2 .
	manualset3
114326	3	403407	5	NULL	NULL	0	NULL	lipid metabolism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Myostatin regulates preadipocyte differentiation and lipid metabolism of adipocyte via ERK1/2 .
	manualset3
114327	4	403407	5	NULL	NULL	0	NULL	adipocyte 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Myostatin regulates preadipocyte differentiation and lipid metabolism of adipocyte via ERK1/2 .
	manualset3
114328	5	403407	5	NULL	NULL	0	NULL	ERK1/2	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Myostatin regulates preadipocyte differentiation and lipid metabolism of adipocyte via ERK1/2 .
	manualset3
114329	1	403408	5	NULL	NULL	0	NULL	N-Acetyl-D-mannosamine ( ManNAc )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	N-Acetyl-D-mannosamine ( ManNAc ) is a specific substrate for the synthesis of N-acetylneuraminic acid , the essential precursor of bacterial capsular polysialic acid ( PA ) .
	manualset3
114330	2	403408	5	NULL	NULL	0	NULL	specific substrate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	N-Acetyl-D-mannosamine ( ManNAc ) is a specific substrate for the synthesis of N-acetylneuraminic acid , the essential precursor of bacterial capsular polysialic acid ( PA ) .
	manualset3
114331	3	403408	5	NULL	NULL	0	NULL	synthesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	N-Acetyl-D-mannosamine ( ManNAc ) is a specific substrate for the synthesis of N-acetylneuraminic acid , the essential precursor of bacterial capsular polysialic acid ( PA ) .
	manualset3
114332	4	403408	5	NULL	NULL	0	NULL	N-acetylneuraminic acid	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	N-Acetyl-D-mannosamine ( ManNAc ) is a specific substrate for the synthesis of N-acetylneuraminic acid , the essential precursor of bacterial capsular polysialic acid ( PA ) .
	manualset3
114333	5	403408	5	NULL	NULL	0	NULL	essential precursor 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	N-Acetyl-D-mannosamine ( ManNAc ) is a specific substrate for the synthesis of N-acetylneuraminic acid , the essential precursor of bacterial capsular polysialic acid ( PA ) .
	manualset3
114334	6	403408	5	NULL	NULL	0	NULL	bacterial capsular polysialic acid ( PA )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	N-Acetyl-D-mannosamine ( ManNAc ) is a specific substrate for the synthesis of N-acetylneuraminic acid , the essential precursor of bacterial capsular polysialic acid ( PA ) .
	manualset3
114335	1	403409	5	NULL	NULL	0	NULL	N-Acetylhistamine deacetylase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	N-Acetylhistamine deacetylase activity increased 80 % in the presence of 1 mM Mn2 + .
	manualset3
114336	2	403409	5	NULL	NULL	0	NULL	 80 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	N-Acetylhistamine deacetylase activity increased 80 % in the presence of 1 mM Mn2 + .
	manualset3
114337	3	403409	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	N-Acetylhistamine deacetylase activity increased 80 % in the presence of 1 mM Mn2 + .
	manualset3
114338	4	403409	5	NULL	NULL	0	NULL	1 mM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	N-Acetylhistamine deacetylase activity increased 80 % in the presence of 1 mM Mn2 + .
	manualset3
114339	5	403409	5	NULL	NULL	0	NULL	Mn2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	N-Acetylhistamine deacetylase activity increased 80 % in the presence of 1 mM Mn2 + .
	manualset3
114340	1	403410	5	NULL	NULL	0	NULL	N-Acetylneuraminic acid nitrogen	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	N-Acetylneuraminic acid nitrogen and thioglycosides were not inducers , whereas 2 , 3-dehydro-N-acetylneuraminic acid , a transition state analog for neuraminidases , was the most effective inductive ligand .
	manualset3
114341	2	403410	5	NULL	NULL	0	NULL	thioglycosides 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	N-Acetylneuraminic acid nitrogen and thioglycosides were not inducers , whereas 2 , 3-dehydro-N-acetylneuraminic acid , a transition state analog for neuraminidases , was the most effective inductive ligand .
	manualset3
114342	3	403410	5	NULL	NULL	0	NULL	inducers 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	N-Acetylneuraminic acid nitrogen and thioglycosides were not inducers , whereas 2 , 3-dehydro-N-acetylneuraminic acid , a transition state analog for neuraminidases , was the most effective inductive ligand .
	manualset3
114343	4	403410	5	NULL	NULL	0	NULL	2 , 3-dehydro-N-acetylneuraminic acid	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	N-Acetylneuraminic acid nitrogen and thioglycosides were not inducers , whereas 2 , 3-dehydro-N-acetylneuraminic acid , a transition state analog for neuraminidases , was the most effective inductive ligand .
	manualset3
114344	5	403410	5	NULL	NULL	0	NULL	transition state analog	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	N-Acetylneuraminic acid nitrogen and thioglycosides were not inducers , whereas 2 , 3-dehydro-N-acetylneuraminic acid , a transition state analog for neuraminidases , was the most effective inductive ligand .
	manualset3
114345	6	403410	5	NULL	NULL	0	NULL	neuraminidases 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	N-Acetylneuraminic acid nitrogen and thioglycosides were not inducers , whereas 2 , 3-dehydro-N-acetylneuraminic acid , a transition state analog for neuraminidases , was the most effective inductive ligand .
	manualset3
114346	7	403410	5	NULL	NULL	0	NULL	effective inductive ligand	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	N-Acetylneuraminic acid nitrogen and thioglycosides were not inducers , whereas 2 , 3-dehydro-N-acetylneuraminic acid , a transition state analog for neuraminidases , was the most effective inductive ligand .
	manualset3
114347	1	403411	5	NULL	NULL	0	NULL	N-Arachidonoylethanolamine ( anandamide ; AEA )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	N-Arachidonoylethanolamine ( anandamide ; AEA ) and 2-arachidonoylglycerol ( 2-AG ) , the two proposed endogenous agonists of cannabinoid receptors , and the putative AEA biosynthetic precursor , N-arachidonoylphosphatidylethanolamine ( NArPE ) , were identified in bovine retina by means of gas chromatography-electron impact mass spectrometry ( GC-EIMS ) .
	manualset3
114348	2	403411	5	NULL	NULL	0	NULL	 2-arachidonoylglycerol ( 2-AG )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	N-Arachidonoylethanolamine ( anandamide ; AEA ) and 2-arachidonoylglycerol ( 2-AG ) , the two proposed endogenous agonists of cannabinoid receptors , and the putative AEA biosynthetic precursor , N-arachidonoylphosphatidylethanolamine ( NArPE ) , were identified in bovine retina by means of gas chromatography-electron impact mass spectrometry ( GC-EIMS ) .
	manualset3
114349	3	403411	5	NULL	NULL	0	NULL	 two	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	N-Arachidonoylethanolamine ( anandamide ; AEA ) and 2-arachidonoylglycerol ( 2-AG ) , the two proposed endogenous agonists of cannabinoid receptors , and the putative AEA biosynthetic precursor , N-arachidonoylphosphatidylethanolamine ( NArPE ) , were identified in bovine retina by means of gas chromatography-electron impact mass spectrometry ( GC-EIMS ) .
	manualset3
114350	4	403411	5	NULL	NULL	0	NULL	endogenous agonists	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	N-Arachidonoylethanolamine ( anandamide ; AEA ) and 2-arachidonoylglycerol ( 2-AG ) , the two proposed endogenous agonists of cannabinoid receptors , and the putative AEA biosynthetic precursor , N-arachidonoylphosphatidylethanolamine ( NArPE ) , were identified in bovine retina by means of gas chromatography-electron impact mass spectrometry ( GC-EIMS ) .
	manualset3
114351	5	403411	5	NULL	NULL	0	NULL	cannabinoid receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	N-Arachidonoylethanolamine ( anandamide ; AEA ) and 2-arachidonoylglycerol ( 2-AG ) , the two proposed endogenous agonists of cannabinoid receptors , and the putative AEA biosynthetic precursor , N-arachidonoylphosphatidylethanolamine ( NArPE ) , were identified in bovine retina by means of gas chromatography-electron impact mass spectrometry ( GC-EIMS ) .
	manualset3
114352	6	403411	5	NULL	NULL	NULL	NULL	putative AEA biosynthetic precursor	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	N-Arachidonoylethanolamine ( anandamide ; AEA ) and 2-arachidonoylglycerol ( 2-AG ) , the two proposed endogenous agonists of cannabinoid receptors , and the putative AEA biosynthetic precursor , N-arachidonoylphosphatidylethanolamine ( NArPE ) , were identified in bovine retina by means of gas chromatography-electron impact mass spectrometry ( GC-EIMS ) .
	manualset3
114353	7	403411	5	NULL	NULL	0	NULL	bovine retina	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	N-Arachidonoylethanolamine ( anandamide ; AEA ) and 2-arachidonoylglycerol ( 2-AG ) , the two proposed endogenous agonists of cannabinoid receptors , and the putative AEA biosynthetic precursor , N-arachidonoylphosphatidylethanolamine ( NArPE ) , were identified in bovine retina by means of gas chromatography-electron impact mass spectrometry ( GC-EIMS ) .
	manualset3
114354	8	403411	5	NULL	NULL	0	NULL	gas chromatography-electron impact mass spectrometry ( GC-EIMS )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	N-Arachidonoylethanolamine ( anandamide ; AEA ) and 2-arachidonoylglycerol ( 2-AG ) , the two proposed endogenous agonists of cannabinoid receptors , and the putative AEA biosynthetic precursor , N-arachidonoylphosphatidylethanolamine ( NArPE ) , were identified in bovine retina by means of gas chromatography-electron impact mass spectrometry ( GC-EIMS ) .
	manualset3
121228	9	403411	5	NULL	NULL	0	NULL	N-arachidonoylphosphatidylethanolamine ( NArPE )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	N-Arachidonoylethanolamine ( anandamide ; AEA ) and 2-arachidonoylglycerol ( 2-AG ) , the two proposed endogenous agonists of cannabinoid receptors , and the putative AEA biosynthetic precursor , N-arachidonoylphosphatidylethanolamine ( NArPE ) , were identified in bovine retina by means of gas chromatography-electron impact mass spectrometry ( GC-EIMS ) .
	manualset3
114394	1	403412	5	NULL	NULL	0	NULL	N-GMSC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	N-GMSC and H-GMSC showed distinct immunoregulatory functions in a murine skin allograft setting via up-regulation of putative systemic regulatory T cells ( Tregs ) .
	manualset3
114396	2	403412	5	NULL	NULL	0	NULL	H-GMSC 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	N-GMSC and H-GMSC showed distinct immunoregulatory functions in a murine skin allograft setting via up-regulation of putative systemic regulatory T cells ( Tregs ) .
	manualset3
114397	3	403412	5	NULL	NULL	0	NULL	immunoregulatory functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	N-GMSC and H-GMSC showed distinct immunoregulatory functions in a murine skin allograft setting via up-regulation of putative systemic regulatory T cells ( Tregs ) .
	manualset3
114398	4	403412	5	NULL	NULL	0	NULL	murine skin allograft	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	N-GMSC and H-GMSC showed distinct immunoregulatory functions in a murine skin allograft setting via up-regulation of putative systemic regulatory T cells ( Tregs ) .
	manualset3
114399	5	403412	5	NULL	NULL	NULL	NULL	up-regulation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	N-GMSC and H-GMSC showed distinct immunoregulatory functions in a murine skin allograft setting via up-regulation of putative systemic regulatory T cells ( Tregs ) .
	manualset3
114400	6	403412	5	NULL	NULL	0	NULL	putative systemic regulatory T cells ( Tregs )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	N-GMSC and H-GMSC showed distinct immunoregulatory functions in a murine skin allograft setting via up-regulation of putative systemic regulatory T cells ( Tregs ) .
	manualset3
114401	1	403413	5	NULL	NULL	0	NULL	N-acetylaspartate ( NAA )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	N-acetylaspartate ( NAA ) , the most prominent signal in proton spectra of normal brain , is a neuron-specific molecule .
	manualset3
114404	2	403413	5	NULL	NULL	0	NULL	prominent signal	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	N-acetylaspartate ( NAA ) , the most prominent signal in proton spectra of normal brain , is a neuron-specific molecule .
	manualset3
114409	3	403413	5	NULL	NULL	0	NULL	proton spectra	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	N-acetylaspartate ( NAA ) , the most prominent signal in proton spectra of normal brain , is a neuron-specific molecule .
	manualset3
114411	4	403413	5	NULL	NULL	0	NULL	normal brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	N-acetylaspartate ( NAA ) , the most prominent signal in proton spectra of normal brain , is a neuron-specific molecule .
	manualset3
114413	5	403413	5	NULL	NULL	0	NULL	neuron-specific molecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	N-acetylaspartate ( NAA ) , the most prominent signal in proton spectra of normal brain , is a neuron-specific molecule .
	manualset3
114416	1	403414	5	NULL	NULL	0	NULL	commentary 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A commentary on neonatology in 1979 .
	manualset3
114417	2	403414	5	NULL	NULL	0	NULL	neonatology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A commentary on neonatology in 1979 .
	manualset3
114419	3	403414	5	NULL	NULL	0	NULL	1979 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	A commentary on neonatology in 1979 .
	manualset3
114426	1	403415	5	NULL	NULL	NULL	NULL	N-alkanes v. ytterbium/faecal index	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	N-alkanes v. ytterbium/faecal index as two methods for estimating herbage intake of dairy cows fed on diets differing in the herbage : maize silage ratio and feeding level .
	manualset3
114427	2	403415	5	NULL	NULL	0	NULL	two	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	N-alkanes v. ytterbium/faecal index as two methods for estimating herbage intake of dairy cows fed on diets differing in the herbage : maize silage ratio and feeding level .
	manualset3
114428	3	403415	5	NULL	NULL	0	NULL	methods 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	N-alkanes v. ytterbium/faecal index as two methods for estimating herbage intake of dairy cows fed on diets differing in the herbage : maize silage ratio and feeding level .
	manualset3
114429	4	403415	5	NULL	NULL	0	NULL	herbage intake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	N-alkanes v. ytterbium/faecal index as two methods for estimating herbage intake of dairy cows fed on diets differing in the herbage : maize silage ratio and feeding level .
	manualset3
114430	5	403415	5	NULL	NULL	0	NULL	dairy cows	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	N-alkanes v. ytterbium/faecal index as two methods for estimating herbage intake of dairy cows fed on diets differing in the herbage : maize silage ratio and feeding level .
	manualset3
114431	6	403415	5	NULL	NULL	0	NULL	diets 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	N-alkanes v. ytterbium/faecal index as two methods for estimating herbage intake of dairy cows fed on diets differing in the herbage : maize silage ratio and feeding level .
	manualset3
114432	7	403415	5	NULL	NULL	0	NULL	herbage 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	N-alkanes v. ytterbium/faecal index as two methods for estimating herbage intake of dairy cows fed on diets differing in the herbage : maize silage ratio and feeding level .
	manualset3
114433	8	403415	5	NULL	NULL	0	NULL	maize silage ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	N-alkanes v. ytterbium/faecal index as two methods for estimating herbage intake of dairy cows fed on diets differing in the herbage : maize silage ratio and feeding level .
	manualset3
114434	9	403415	5	NULL	NULL	0	NULL	feeding level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	N-alkanes v. ytterbium/faecal index as two methods for estimating herbage intake of dairy cows fed on diets differing in the herbage : maize silage ratio and feeding level .
	manualset3
114435	1	403416	5	NULL	NULL	0	NULL	N-glycanase treatment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	N-glycanase treatment cleaved the oligosaccharide from the G-pPRLs , establishing N-linked glycosylation .
	manualset3
114436	2	403416	5	NULL	NULL	0	NULL	oligosaccharide 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	N-glycanase treatment cleaved the oligosaccharide from the G-pPRLs , establishing N-linked glycosylation .
	manualset3
114437	3	403416	5	NULL	NULL	0	NULL	G-pPRLs	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	N-glycanase treatment cleaved the oligosaccharide from the G-pPRLs , establishing N-linked glycosylation .
	manualset3
114438	4	403416	5	NULL	NULL	0	NULL	N-linked glycosylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	N-glycanase treatment cleaved the oligosaccharide from the G-pPRLs , establishing N-linked glycosylation .
	manualset3
114439	1	403417	5	NULL	NULL	0	NULL	N-glycosylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	N-glycosylation of ECL1 caused a very significant decrease in affinity and cell surface expression of the resulting receptor .
	manualset3
114440	2	403417	5	NULL	NULL	0	NULL	ECL1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	N-glycosylation of ECL1 caused a very significant decrease in affinity and cell surface expression of the resulting receptor .
	manualset3
114441	3	403417	5	NULL	NULL	NULL	NULL	affinity 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	N-glycosylation of ECL1 caused a very significant decrease in affinity and cell surface expression of the resulting receptor .
	manualset3
114442	4	403417	5	NULL	NULL	0	NULL	cell surface expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	N-glycosylation of ECL1 caused a very significant decrease in affinity and cell surface expression of the resulting receptor .
	manualset3
114443	5	403417	5	NULL	NULL	0	NULL	receptor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	N-glycosylation of ECL1 caused a very significant decrease in affinity and cell surface expression of the resulting receptor .
	manualset3
114444	1	403418	5	NULL	NULL	0	NULL	N-hydroxyformamide peptidomimetics	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	N-hydroxyformamide peptidomimetics as TACE/matrix metalloprotease inhibitors : oral activity via P1 ' isobutyl substitution .
	manualset3
114445	2	403418	5	NULL	NULL	0	NULL	TACE/matrix metalloprotease inhibitors	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	N-hydroxyformamide peptidomimetics as TACE/matrix metalloprotease inhibitors : oral activity via P1 ' isobutyl substitution .
	manualset3
114446	3	403418	5	NULL	NULL	0	NULL	oral activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	N-hydroxyformamide peptidomimetics as TACE/matrix metalloprotease inhibitors : oral activity via P1 ' isobutyl substitution .
	manualset3
114447	4	403418	5	NULL	NULL	0	NULL	P1 ' isobutyl substitution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	N-hydroxyformamide peptidomimetics as TACE/matrix metalloprotease inhibitors : oral activity via P1 ' isobutyl substitution .
	manualset3
114448	1	403419	5	NULL	NULL	0	NULL	N-terminal domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	N-terminal domains of DELLA proteins are intrinsically unstructured in the absence of interaction with GID1/gibberellic acid receptors .
	manualset3
114449	2	403419	5	NULL	NULL	0	NULL	DELLA proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	N-terminal domains of DELLA proteins are intrinsically unstructured in the absence of interaction with GID1/gibberellic acid receptors .
	manualset3
114450	3	403419	5	NULL	NULL	0	NULL	absence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	N-terminal domains of DELLA proteins are intrinsically unstructured in the absence of interaction with GID1/gibberellic acid receptors .
	manualset3
114451	4	403419	5	NULL	NULL	0	NULL	interaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	N-terminal domains of DELLA proteins are intrinsically unstructured in the absence of interaction with GID1/gibberellic acid receptors .
	manualset3
114452	5	403419	5	NULL	NULL	0	NULL	GID1/gibberellic acid receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	N-terminal domains of DELLA proteins are intrinsically unstructured in the absence of interaction with GID1/gibberellic acid receptors .
	manualset3
114453	1	403420	5	NULL	NULL	0	NULL	N - ( 3 - ( 3 - ( 1-Piperidinylmethyl ) phenoxy ) propyl ) - acetoxyacetamide + + + hydrochloride ( TZU-0460 ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	N - ( 3 - ( 3 - ( 1-Piperidinylmethyl ) phenoxy ) propyl ) - acetoxyacetamide + + + hydrochloride ( TZU-0460 ) was compared with cimetidine for the effects on gastric acid secretion in dog and rat and on ulcer formation in rat .
	manualset3
114454	2	403420	5	NULL	NULL	0	NULL	cimetidine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	N - ( 3 - ( 3 - ( 1-Piperidinylmethyl ) phenoxy ) propyl ) - acetoxyacetamide + + + hydrochloride ( TZU-0460 ) was compared with cimetidine for the effects on gastric acid secretion in dog and rat and on ulcer formation in rat .
	manualset3
114455	3	403420	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	N - ( 3 - ( 3 - ( 1-Piperidinylmethyl ) phenoxy ) propyl ) - acetoxyacetamide + + + hydrochloride ( TZU-0460 ) was compared with cimetidine for the effects on gastric acid secretion in dog and rat and on ulcer formation in rat .
	manualset3
114456	4	403420	5	NULL	NULL	0	NULL	gastric acid secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	N - ( 3 - ( 3 - ( 1-Piperidinylmethyl ) phenoxy ) propyl ) - acetoxyacetamide + + + hydrochloride ( TZU-0460 ) was compared with cimetidine for the effects on gastric acid secretion in dog and rat and on ulcer formation in rat .
	manualset3
114457	5	403420	5	NULL	NULL	0	NULL	dog 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	N - ( 3 - ( 3 - ( 1-Piperidinylmethyl ) phenoxy ) propyl ) - acetoxyacetamide + + + hydrochloride ( TZU-0460 ) was compared with cimetidine for the effects on gastric acid secretion in dog and rat and on ulcer formation in rat .
	manualset3
114458	6	403420	5	NULL	NULL	0	NULL	rat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	N - ( 3 - ( 3 - ( 1-Piperidinylmethyl ) phenoxy ) propyl ) - acetoxyacetamide + + + hydrochloride ( TZU-0460 ) was compared with cimetidine for the effects on gastric acid secretion in dog and rat and on ulcer formation in rat .
	manualset3
114459	7	403420	5	NULL	NULL	0	NULL	ulcer formation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	N - ( 3 - ( 3 - ( 1-Piperidinylmethyl ) phenoxy ) propyl ) - acetoxyacetamide + + + hydrochloride ( TZU-0460 ) was compared with cimetidine for the effects on gastric acid secretion in dog and rat and on ulcer formation in rat .
	manualset3
114460	8	403420	5	NULL	NULL	0	NULL	rat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	N - ( 3 - ( 3 - ( 1-Piperidinylmethyl ) phenoxy ) propyl ) - acetoxyacetamide + + + hydrochloride ( TZU-0460 ) was compared with cimetidine for the effects on gastric acid secretion in dog and rat and on ulcer formation in rat .
	manualset3
114461	1	403421	5	NULL	NULL	0	NULL	N - ( 4-Methyl-benzo-yl ) -4 - nitro-benzene-sulfonamide	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	N - ( 4-Methyl-benzo-yl ) -4 - nitro-benzene-sulfonamide .
	manualset3
114462	1	403422	5	NULL	NULL	0	NULL	N - ( 7-Nitrobenzofurazan-4-yl ) taurine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	N - ( 7-Nitrobenzofurazan-4-yl ) taurine , a fluorescent substrate-analogue of the system .
	manualset3
114463	2	403422	5	NULL	NULL	0	NULL	fluorescent substrate-analogue	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	N - ( 7-Nitrobenzofurazan-4-yl ) taurine , a fluorescent substrate-analogue of the system .
	manualset3
114464	3	403422	5	NULL	NULL	0	NULL	system 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	N - ( 7-Nitrobenzofurazan-4-yl ) taurine , a fluorescent substrate-analogue of the system .
	manualset3
114465	1	403423	5	NULL	NULL	0	NULL	NAD ( P ) H oxidase inhibitors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	NAD ( P ) H oxidase inhibitors prevented H2O2 generation and DNA ladder formation .
	manualset3
114466	2	403423	5	NULL	NULL	0	NULL	H2O2 generation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	NAD ( P ) H oxidase inhibitors prevented H2O2 generation and DNA ladder formation .
	manualset3
114467	3	403423	5	NULL	NULL	0	NULL	DNA ladder formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	NAD ( P ) H oxidase inhibitors prevented H2O2 generation and DNA ladder formation .
	manualset3
114468	1	403424	5	NULL	NULL	0	NULL	NADP ( H ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	NADP ( H ) , which is confined in the protein complex , was oxidized or reduced during the enzymatic reactions and the changes in the fluorescence intensity were related to the substrate concentration .
	manualset3
114469	2	403424	5	NULL	NULL	0	NULL	protein complex 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	NADP ( H ) , which is confined in the protein complex , was oxidized or reduced during the enzymatic reactions and the changes in the fluorescence intensity were related to the substrate concentration .
	manualset3
114470	3	403424	5	NULL	NULL	0	NULL	enzymatic reactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	NADP ( H ) , which is confined in the protein complex , was oxidized or reduced during the enzymatic reactions and the changes in the fluorescence intensity were related to the substrate concentration .
	manualset3
114471	4	403424	5	NULL	NULL	NULL	NULL	changes 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	NADP ( H ) , which is confined in the protein complex , was oxidized or reduced during the enzymatic reactions and the changes in the fluorescence intensity were related to the substrate concentration .
	manualset3
114472	5	403424	5	NULL	NULL	0	NULL	fluorescence intensity 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	NADP ( H ) , which is confined in the protein complex , was oxidized or reduced during the enzymatic reactions and the changes in the fluorescence intensity were related to the substrate concentration .
	manualset3
114473	6	403424	5	NULL	NULL	0	NULL	substrate concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	NADP ( H ) , which is confined in the protein complex , was oxidized or reduced during the enzymatic reactions and the changes in the fluorescence intensity were related to the substrate concentration .
	manualset3
114474	1	403425	5	NULL	NULL	0	NULL	NADPH-diaphorase expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	NADPH-diaphorase expression of endothelial cells during four weeks ' healing of a stretch-ePTFE graft : an experimental porcine study .
	manualset3
114475	2	403425	5	NULL	NULL	0	NULL	endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	NADPH-diaphorase expression of endothelial cells during four weeks ' healing of a stretch-ePTFE graft : an experimental porcine study .
	manualset3
114476	3	403425	5	NULL	NULL	0	NULL	 four weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	NADPH-diaphorase expression of endothelial cells during four weeks ' healing of a stretch-ePTFE graft : an experimental porcine study .
	manualset3
114477	4	403425	5	NULL	NULL	0	NULL	healing 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	NADPH-diaphorase expression of endothelial cells during four weeks ' healing of a stretch-ePTFE graft : an experimental porcine study .
	manualset3
114478	5	403425	5	NULL	NULL	0	NULL	stretch-ePTFE graft	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	NADPH-diaphorase expression of endothelial cells during four weeks ' healing of a stretch-ePTFE graft : an experimental porcine study .
	manualset3
114479	6	403425	5	NULL	NULL	0	NULL	experimental porcine study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	NADPH-diaphorase expression of endothelial cells during four weeks ' healing of a stretch-ePTFE graft : an experimental porcine study .
	manualset3
114480	1	403426	5	NULL	NULL	0	NULL	NCI-60 anticancer screening assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	NCI-60 anticancer screening assays showed that thailandepsins possess broad-spectrum antiproliferative activities with GI50 for over 90 % of the tested cell lines at low nanomolar concentrations and potent cytotoxic activities toward certain types of cell lines , particularly for those derived from colon , melanoma , ovarian , and renal cancers .
	manualset3
114521	2	403426	5	NULL	NULL	0	NULL	thailandepsins	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	NCI-60 anticancer screening assays showed that thailandepsins possess broad-spectrum antiproliferative activities with GI50 for over 90 % of the tested cell lines at low nanomolar concentrations and potent cytotoxic activities toward certain types of cell lines , particularly for those derived from colon , melanoma , ovarian , and renal cancers .
	manualset3
114522	3	403426	5	NULL	NULL	0	NULL	broad-spectrum antiproliferative activities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	NCI-60 anticancer screening assays showed that thailandepsins possess broad-spectrum antiproliferative activities with GI50 for over 90 % of the tested cell lines at low nanomolar concentrations and potent cytotoxic activities toward certain types of cell lines , particularly for those derived from colon , melanoma , ovarian , and renal cancers .
	manualset3
114523	4	403426	5	NULL	NULL	0	NULL	GI50	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	NCI-60 anticancer screening assays showed that thailandepsins possess broad-spectrum antiproliferative activities with GI50 for over 90 % of the tested cell lines at low nanomolar concentrations and potent cytotoxic activities toward certain types of cell lines , particularly for those derived from colon , melanoma , ovarian , and renal cancers .
	manualset3
114524	5	403426	5	NULL	NULL	0	NULL	90 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	NCI-60 anticancer screening assays showed that thailandepsins possess broad-spectrum antiproliferative activities with GI50 for over 90 % of the tested cell lines at low nanomolar concentrations and potent cytotoxic activities toward certain types of cell lines , particularly for those derived from colon , melanoma , ovarian , and renal cancers .
	manualset3
114525	6	403426	5	NULL	NULL	0	NULL	tested cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	NCI-60 anticancer screening assays showed that thailandepsins possess broad-spectrum antiproliferative activities with GI50 for over 90 % of the tested cell lines at low nanomolar concentrations and potent cytotoxic activities toward certain types of cell lines , particularly for those derived from colon , melanoma , ovarian , and renal cancers .
	manualset3
114526	7	403426	5	NULL	NULL	0	NULL	low nanomolar concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	NCI-60 anticancer screening assays showed that thailandepsins possess broad-spectrum antiproliferative activities with GI50 for over 90 % of the tested cell lines at low nanomolar concentrations and potent cytotoxic activities toward certain types of cell lines , particularly for those derived from colon , melanoma , ovarian , and renal cancers .
	manualset3
114527	8	403426	5	NULL	NULL	0	NULL	potent cytotoxic activities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	NCI-60 anticancer screening assays showed that thailandepsins possess broad-spectrum antiproliferative activities with GI50 for over 90 % of the tested cell lines at low nanomolar concentrations and potent cytotoxic activities toward certain types of cell lines , particularly for those derived from colon , melanoma , ovarian , and renal cancers .
	manualset3
114528	9	403426	5	NULL	NULL	0	NULL	certain types	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	NCI-60 anticancer screening assays showed that thailandepsins possess broad-spectrum antiproliferative activities with GI50 for over 90 % of the tested cell lines at low nanomolar concentrations and potent cytotoxic activities toward certain types of cell lines , particularly for those derived from colon , melanoma , ovarian , and renal cancers .
	manualset3
114529	10	403426	5	NULL	NULL	0	NULL	cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	NCI-60 anticancer screening assays showed that thailandepsins possess broad-spectrum antiproliferative activities with GI50 for over 90 % of the tested cell lines at low nanomolar concentrations and potent cytotoxic activities toward certain types of cell lines , particularly for those derived from colon , melanoma , ovarian , and renal cancers .
	manualset3
114530	11	403426	5	NULL	NULL	0	NULL	colon cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	NCI-60 anticancer screening assays showed that thailandepsins possess broad-spectrum antiproliferative activities with GI50 for over 90 % of the tested cell lines at low nanomolar concentrations and potent cytotoxic activities toward certain types of cell lines , particularly for those derived from colon , melanoma , ovarian , and renal cancers .
	manualset3
114531	12	403426	5	NULL	NULL	0	NULL	melanoma cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	NCI-60 anticancer screening assays showed that thailandepsins possess broad-spectrum antiproliferative activities with GI50 for over 90 % of the tested cell lines at low nanomolar concentrations and potent cytotoxic activities toward certain types of cell lines , particularly for those derived from colon , melanoma , ovarian , and renal cancers .
	manualset3
114532	13	403426	5	NULL	NULL	0	NULL	ovarian cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	NCI-60 anticancer screening assays showed that thailandepsins possess broad-spectrum antiproliferative activities with GI50 for over 90 % of the tested cell lines at low nanomolar concentrations and potent cytotoxic activities toward certain types of cell lines , particularly for those derived from colon , melanoma , ovarian , and renal cancers .
	manualset3
114533	14	403426	5	NULL	NULL	0	NULL	renal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	NCI-60 anticancer screening assays showed that thailandepsins possess broad-spectrum antiproliferative activities with GI50 for over 90 % of the tested cell lines at low nanomolar concentrations and potent cytotoxic activities toward certain types of cell lines , particularly for those derived from colon , melanoma , ovarian , and renal cancers .
	manualset3
114534	1	403427	5	NULL	NULL	0	NULL	NE	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	NE , E and DBH were found not to reflect tumor activity .
	manualset3
114535	2	403427	5	NULL	NULL	0	NULL	E	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	NE , E and DBH were found not to reflect tumor activity .
	manualset3
114536	3	403427	5	NULL	NULL	0	NULL	DBH	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	NE , E and DBH were found not to reflect tumor activity .
	manualset3
114537	4	403427	5	NULL	NULL	0	NULL	tumor activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	NE , E and DBH were found not to reflect tumor activity .
	manualset3
114538	1	403428	5	NULL	NULL	0	NULL	PHYSIOLOGICAL TESTING METHODS	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	NEW PHYSIOLOGICAL TESTING METHODS AVAILABLE TO UROLOGISTS .
	manualset3
114539	2	403428	5	NULL	NULL	0	NULL	UROLOGISTS	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	NEW PHYSIOLOGICAL TESTING METHODS AVAILABLE TO UROLOGISTS .
	manualset3
114540	1	403429	5	NULL	NULL	0	NULL	Bioactive molecular forms	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Bioactive and immunoreactive molecular forms of adrenocorticotropic hormone in the fetal rat hypophysis ( author 's transl ) ) .
	manualset3
114541	2	403429	5	NULL	NULL	0	NULL	immunoreactive molecular forms	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Bioactive and immunoreactive molecular forms of adrenocorticotropic hormone in the fetal rat hypophysis ( author 's transl ) ) .
	manualset3
114542	3	403429	5	NULL	NULL	0	NULL	adrenocorticotropic hormone	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Bioactive and immunoreactive molecular forms of adrenocorticotropic hormone in the fetal rat hypophysis ( author 's transl ) ) .
	manualset3
114543	4	403429	5	NULL	NULL	0	NULL	fetal rat hypophysis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Bioactive and immunoreactive molecular forms of adrenocorticotropic hormone in the fetal rat hypophysis ( author 's transl ) ) .
	manualset3
114544	1	403430	5	NULL	NULL	0	NULL	NFBD1/MDC1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	NFBD1/MDC1 regulates Cav1 and Cav2 independently of DNA damage and p53 .
	manualset3
114545	2	403430	5	NULL	NULL	0	NULL	Cav1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	NFBD1/MDC1 regulates Cav1 and Cav2 independently of DNA damage and p53 .
	manualset3
114546	3	403430	5	NULL	NULL	0	NULL	Cav2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	NFBD1/MDC1 regulates Cav1 and Cav2 independently of DNA damage and p53 .
	manualset3
114547	4	403430	5	NULL	NULL	0	NULL	DNA damage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	NFBD1/MDC1 regulates Cav1 and Cav2 independently of DNA damage and p53 .
	manualset3
114548	5	403430	5	NULL	NULL	0	NULL	p53	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	NFBD1/MDC1 regulates Cav1 and Cav2 independently of DNA damage and p53 .
	manualset3
114549	1	403431	5	NULL	NULL	0	NULL	NGF-induced activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	NGF-induced activation of PKC-iota was observed to be dependent on phosphatidylinositol 3-kinase ( PI3K ) and led to coassociation of PKC-iota with Ras and Src .
	manualset3
114550	2	403431	5	NULL	NULL	0	NULL	PKC-iota	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	NGF-induced activation of PKC-iota was observed to be dependent on phosphatidylinositol 3-kinase ( PI3K ) and led to coassociation of PKC-iota with Ras and Src .
	manualset3
114551	3	403431	5	NULL	NULL	0	NULL	phosphatidylinositol 3-kinase ( PI3K )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	NGF-induced activation of PKC-iota was observed to be dependent on phosphatidylinositol 3-kinase ( PI3K ) and led to coassociation of PKC-iota with Ras and Src .
	manualset3
114552	4	403431	5	NULL	NULL	0	NULL	coassociation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	NGF-induced activation of PKC-iota was observed to be dependent on phosphatidylinositol 3-kinase ( PI3K ) and led to coassociation of PKC-iota with Ras and Src .
	manualset3
114553	5	403431	5	NULL	NULL	0	NULL	PKC-iota	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	NGF-induced activation of PKC-iota was observed to be dependent on phosphatidylinositol 3-kinase ( PI3K ) and led to coassociation of PKC-iota with Ras and Src .
	manualset3
114554	6	403431	5	NULL	NULL	0	NULL	Ras	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	NGF-induced activation of PKC-iota was observed to be dependent on phosphatidylinositol 3-kinase ( PI3K ) and led to coassociation of PKC-iota with Ras and Src .
	manualset3
114555	7	403431	5	NULL	NULL	0	NULL	Src	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	NGF-induced activation of PKC-iota was observed to be dependent on phosphatidylinositol 3-kinase ( PI3K ) and led to coassociation of PKC-iota with Ras and Src .
	manualset3
114556	1	403432	5	NULL	NULL	0	NULL	NH concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	NH and AH concentrations were obtained by serial dilution with tryptic soy broth ( TSB ) .
	manualset3
114557	2	403432	5	NULL	NULL	0	NULL	AH concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	NH and AH concentrations were obtained by serial dilution with tryptic soy broth ( TSB ) .
	manualset3
114558	3	403432	5	NULL	NULL	0	NULL	serial dilution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	NH and AH concentrations were obtained by serial dilution with tryptic soy broth ( TSB ) .
	manualset3
114559	4	403432	5	NULL	NULL	0	NULL	tryptic soy broth ( TSB ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	NH and AH concentrations were obtained by serial dilution with tryptic soy broth ( TSB ) .
	manualset3
114560	1	403433	5	NULL	NULL	0	NULL	NHE1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	NHE1 also regulates formation of invadopodia - cell structures that mediate tumor cell migration and invasion .
	manualset3
114561	2	403433	5	NULL	NULL	0	NULL	formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	NHE1 also regulates formation of invadopodia - cell structures that mediate tumor cell migration and invasion .
	manualset3
114562	3	403433	5	NULL	NULL	0	NULL	invadopodia - cell structures	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	NHE1 also regulates formation of invadopodia - cell structures that mediate tumor cell migration and invasion .
	manualset3
114563	4	403433	5	NULL	NULL	0	NULL	tumor cell migration	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	NHE1 also regulates formation of invadopodia - cell structures that mediate tumor cell migration and invasion .
	manualset3
114564	5	403433	5	NULL	NULL	0	NULL	invasion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	NHE1 also regulates formation of invadopodia - cell structures that mediate tumor cell migration and invasion .
	manualset3
114565	1	403434	5	NULL	NULL	0	NULL	NHS	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	NHS ` vulnerable to racism ' claim .
	manualset3
114566	2	403434	5	NULL	NULL	0	NULL	racism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	NHS ` vulnerable to racism ' claim .
	manualset3
114567	3	403434	5	NULL	NULL	0	NULL	claim	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	NHS ` vulnerable to racism ' claim .
	manualset3
114568	1	403435	5	NULL	NULL	0	NULL	NIRF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	NIRF is a nuclear protein with a ubiquitin-like domain , a PHD finger , a YDG/SRA domain , Rb-binding motifs and a RING finger .
	manualset3
114569	2	403435	5	NULL	NULL	0	NULL	nuclear protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	NIRF is a nuclear protein with a ubiquitin-like domain , a PHD finger , a YDG/SRA domain , Rb-binding motifs and a RING finger .
	manualset3
114570	3	403435	5	NULL	NULL	0	NULL	ubiquitin-like domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	NIRF is a nuclear protein with a ubiquitin-like domain , a PHD finger , a YDG/SRA domain , Rb-binding motifs and a RING finger .
	manualset3
114571	4	403435	5	NULL	NULL	0	NULL	PHD finger	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	NIRF is a nuclear protein with a ubiquitin-like domain , a PHD finger , a YDG/SRA domain , Rb-binding motifs and a RING finger .
	manualset3
114572	5	403435	5	NULL	NULL	0	NULL	YDG/SRA domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	NIRF is a nuclear protein with a ubiquitin-like domain , a PHD finger , a YDG/SRA domain , Rb-binding motifs and a RING finger .
	manualset3
114573	6	403435	5	NULL	NULL	0	NULL	Rb-binding motifs	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	NIRF is a nuclear protein with a ubiquitin-like domain , a PHD finger , a YDG/SRA domain , Rb-binding motifs and a RING finger .
	manualset3
114574	7	403435	5	NULL	NULL	0	NULL	RING finger	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	NIRF is a nuclear protein with a ubiquitin-like domain , a PHD finger , a YDG/SRA domain , Rb-binding motifs and a RING finger .
	manualset3
114575	1	403436	5	NULL	NULL	0	NULL	NK cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	NK cells developed in and were lost from the uteri of pregnant Fas antigen-deficient lpr/lpr mice .
	manualset3
114576	2	403436	5	NULL	NULL	0	NULL	uteri	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	NK cells developed in and were lost from the uteri of pregnant Fas antigen-deficient lpr/lpr mice .
	manualset3
114577	3	403436	5	NULL	NULL	0	NULL	pregnant Fas antigen-deficient lpr/lpr mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	NK cells developed in and were lost from the uteri of pregnant Fas antigen-deficient lpr/lpr mice .
	manualset3
114578	1	403437	5	NULL	NULL	0	NULL	NM23HI	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	NM23HI as marker of metastasis in invasive ductal breast cancer .
	manualset3
114579	2	403437	5	NULL	NULL	0	NULL	marker	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	NM23HI as marker of metastasis in invasive ductal breast cancer .
	manualset3
114580	3	403437	5	NULL	NULL	0	NULL	metastasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	NM23HI as marker of metastasis in invasive ductal breast cancer .
	manualset3
114581	4	403437	5	NULL	NULL	0	NULL	invasive ductal breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	NM23HI as marker of metastasis in invasive ductal breast cancer .
	manualset3
114582	1	403438	5	NULL	NULL	0	NULL	NMR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR and CD characterisation of the denatured states from which fibrils form at low pH show that their properties can be correlated with the nature of the resulting aggregates defined by EM and FTIR spectroscopy .
	manualset3
114583	2	403438	5	NULL	NULL	0	NULL	CD characterisation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR and CD characterisation of the denatured states from which fibrils form at low pH show that their properties can be correlated with the nature of the resulting aggregates defined by EM and FTIR spectroscopy .
	manualset3
114584	3	403438	5	NULL	NULL	0	NULL	denatured states	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR and CD characterisation of the denatured states from which fibrils form at low pH show that their properties can be correlated with the nature of the resulting aggregates defined by EM and FTIR spectroscopy .
	manualset3
114585	4	403438	5	NULL	NULL	0	NULL	fibrils	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR and CD characterisation of the denatured states from which fibrils form at low pH show that their properties can be correlated with the nature of the resulting aggregates defined by EM and FTIR spectroscopy .
	manualset3
114586	5	403438	5	NULL	NULL	0	NULL	low pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR and CD characterisation of the denatured states from which fibrils form at low pH show that their properties can be correlated with the nature of the resulting aggregates defined by EM and FTIR spectroscopy .
	manualset3
114587	6	403438	5	NULL	NULL	0	NULL	properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR and CD characterisation of the denatured states from which fibrils form at low pH show that their properties can be correlated with the nature of the resulting aggregates defined by EM and FTIR spectroscopy .
	manualset3
114588	7	403438	5	NULL	NULL	0	NULL	nature	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR and CD characterisation of the denatured states from which fibrils form at low pH show that their properties can be correlated with the nature of the resulting aggregates defined by EM and FTIR spectroscopy .
	manualset3
114589	8	403438	5	NULL	NULL	0	NULL	resulting aggregates	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR and CD characterisation of the denatured states from which fibrils form at low pH show that their properties can be correlated with the nature of the resulting aggregates defined by EM and FTIR spectroscopy .
	manualset3
114590	9	403438	5	NULL	NULL	0	NULL	EM spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR and CD characterisation of the denatured states from which fibrils form at low pH show that their properties can be correlated with the nature of the resulting aggregates defined by EM and FTIR spectroscopy .
	manualset3
114591	10	403438	5	NULL	NULL	0	NULL	FTIR spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR and CD characterisation of the denatured states from which fibrils form at low pH show that their properties can be correlated with the nature of the resulting aggregates defined by EM and FTIR spectroscopy .
	manualset3
114592	1	403439	5	NULL	NULL	0	NULL	NMR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR and molecular modelling studies of the binding of amicetin antibiotic to conserved secondary structural motifs of 23S ribosomal RNAs .
	manualset3
114593	2	403439	5	NULL	NULL	0	NULL	molecular modelling studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR and molecular modelling studies of the binding of amicetin antibiotic to conserved secondary structural motifs of 23S ribosomal RNAs .
	manualset3
114594	3	403439	5	NULL	NULL	0	NULL	amicetin antibiotic	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR and molecular modelling studies of the binding of amicetin antibiotic to conserved secondary structural motifs of 23S ribosomal RNAs .
	manualset3
114595	4	403439	5	NULL	NULL	NULL	NULL	conserved secondary structural motifs	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	NMR and molecular modelling studies of the binding of amicetin antibiotic to conserved secondary structural motifs of 23S ribosomal RNAs .
	manualset3
114596	5	403439	5	NULL	NULL	0	NULL	23S ribosomal RNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR and molecular modelling studies of the binding of amicetin antibiotic to conserved secondary structural motifs of 23S ribosomal RNAs .
	manualset3
114597	1	403440	5	NULL	NULL	0	NULL	NMR measurements	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR measurements showed an accumulation of glucose-6-phosphate ( G-6-P ) during the ischaemic period , indicating anaerobic metabolism .
	manualset3
114598	2	403440	5	NULL	NULL	0	NULL	accumulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR measurements showed an accumulation of glucose-6-phosphate ( G-6-P ) during the ischaemic period , indicating anaerobic metabolism .
	manualset3
114599	3	403440	5	NULL	NULL	0	NULL	glucose-6-phosphate ( G-6-P )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR measurements showed an accumulation of glucose-6-phosphate ( G-6-P ) during the ischaemic period , indicating anaerobic metabolism .
	manualset3
114600	4	403440	5	NULL	NULL	0	NULL	ischaemic period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR measurements showed an accumulation of glucose-6-phosphate ( G-6-P ) during the ischaemic period , indicating anaerobic metabolism .
	manualset3
114601	5	403440	5	NULL	NULL	0	NULL	anaerobic metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR measurements showed an accumulation of glucose-6-phosphate ( G-6-P ) during the ischaemic period , indicating anaerobic metabolism .
	manualset3
114602	1	403441	5	NULL	NULL	0	NULL	NMR semiselective spin-lattice relaxation rate measurements	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR semiselective spin-lattice relaxation rate measurements and HPLC size-exclusion chromatography studies show that in 20 mM potassium phosphate ( pH 7 ) buffer ( KP ) TET4 is approximately twice the length of the form obtained in 20 mM sodium phosphate ( pH 7 ) buffer ( NaP ) and that mixtures of Na + and K + produce mixtures of the two forms whose populations depend on the ratio of the cations .
	manualset3
114603	2	403441	5	NULL	NULL	0	NULL	HPLC size-exclusion chromatography studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR semiselective spin-lattice relaxation rate measurements and HPLC size-exclusion chromatography studies show that in 20 mM potassium phosphate ( pH 7 ) buffer ( KP ) TET4 is approximately twice the length of the form obtained in 20 mM sodium phosphate ( pH 7 ) buffer ( NaP ) and that mixtures of Na + and K + produce mixtures of the two forms whose populations depend on the ratio of the cations .
	manualset3
114604	3	403441	5	NULL	NULL	0	NULL	20 mM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR semiselective spin-lattice relaxation rate measurements and HPLC size-exclusion chromatography studies show that in 20 mM potassium phosphate ( pH 7 ) buffer ( KP ) TET4 is approximately twice the length of the form obtained in 20 mM sodium phosphate ( pH 7 ) buffer ( NaP ) and that mixtures of Na + and K + produce mixtures of the two forms whose populations depend on the ratio of the cations .
	manualset3
114605	4	403441	5	NULL	NULL	NULL	NULL	potassium phosphate ( pH 7 ) buffer ( KP )	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	NMR semiselective spin-lattice relaxation rate measurements and HPLC size-exclusion chromatography studies show that in 20 mM potassium phosphate ( pH 7 ) buffer ( KP ) TET4 is approximately twice the length of the form obtained in 20 mM sodium phosphate ( pH 7 ) buffer ( NaP ) and that mixtures of Na + and K + produce mixtures of the two forms whose populations depend on the ratio of the cations .
	manualset3
114606	5	403441	5	NULL	NULL	0	NULL	TET4	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR semiselective spin-lattice relaxation rate measurements and HPLC size-exclusion chromatography studies show that in 20 mM potassium phosphate ( pH 7 ) buffer ( KP ) TET4 is approximately twice the length of the form obtained in 20 mM sodium phosphate ( pH 7 ) buffer ( NaP ) and that mixtures of Na + and K + produce mixtures of the two forms whose populations depend on the ratio of the cations .
	manualset3
114607	6	403441	5	NULL	NULL	0	NULL	approximately twice	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR semiselective spin-lattice relaxation rate measurements and HPLC size-exclusion chromatography studies show that in 20 mM potassium phosphate ( pH 7 ) buffer ( KP ) TET4 is approximately twice the length of the form obtained in 20 mM sodium phosphate ( pH 7 ) buffer ( NaP ) and that mixtures of Na + and K + produce mixtures of the two forms whose populations depend on the ratio of the cations .
	manualset3
114608	7	403441	5	NULL	NULL	0	NULL	length	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR semiselective spin-lattice relaxation rate measurements and HPLC size-exclusion chromatography studies show that in 20 mM potassium phosphate ( pH 7 ) buffer ( KP ) TET4 is approximately twice the length of the form obtained in 20 mM sodium phosphate ( pH 7 ) buffer ( NaP ) and that mixtures of Na + and K + produce mixtures of the two forms whose populations depend on the ratio of the cations .
	manualset3
114609	8	403441	5	NULL	NULL	0	NULL	form	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR semiselective spin-lattice relaxation rate measurements and HPLC size-exclusion chromatography studies show that in 20 mM potassium phosphate ( pH 7 ) buffer ( KP ) TET4 is approximately twice the length of the form obtained in 20 mM sodium phosphate ( pH 7 ) buffer ( NaP ) and that mixtures of Na + and K + produce mixtures of the two forms whose populations depend on the ratio of the cations .
	manualset3
114610	9	403441	5	NULL	NULL	0	NULL	20 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR semiselective spin-lattice relaxation rate measurements and HPLC size-exclusion chromatography studies show that in 20 mM potassium phosphate ( pH 7 ) buffer ( KP ) TET4 is approximately twice the length of the form obtained in 20 mM sodium phosphate ( pH 7 ) buffer ( NaP ) and that mixtures of Na + and K + produce mixtures of the two forms whose populations depend on the ratio of the cations .
	manualset3
114611	10	403441	5	NULL	NULL	0	NULL	sodium phosphate ( pH 7 ) buffer ( NaP )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR semiselective spin-lattice relaxation rate measurements and HPLC size-exclusion chromatography studies show that in 20 mM potassium phosphate ( pH 7 ) buffer ( KP ) TET4 is approximately twice the length of the form obtained in 20 mM sodium phosphate ( pH 7 ) buffer ( NaP ) and that mixtures of Na + and K + produce mixtures of the two forms whose populations depend on the ratio of the cations .
	manualset3
114612	11	403441	5	NULL	NULL	0	NULL	mixtures	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR semiselective spin-lattice relaxation rate measurements and HPLC size-exclusion chromatography studies show that in 20 mM potassium phosphate ( pH 7 ) buffer ( KP ) TET4 is approximately twice the length of the form obtained in 20 mM sodium phosphate ( pH 7 ) buffer ( NaP ) and that mixtures of Na + and K + produce mixtures of the two forms whose populations depend on the ratio of the cations .
	manualset3
114613	12	403441	5	NULL	NULL	0	NULL	Na +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR semiselective spin-lattice relaxation rate measurements and HPLC size-exclusion chromatography studies show that in 20 mM potassium phosphate ( pH 7 ) buffer ( KP ) TET4 is approximately twice the length of the form obtained in 20 mM sodium phosphate ( pH 7 ) buffer ( NaP ) and that mixtures of Na + and K + produce mixtures of the two forms whose populations depend on the ratio of the cations .
	manualset3
114620	13	403441	5	NULL	NULL	0	NULL	K +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR semiselective spin-lattice relaxation rate measurements and HPLC size-exclusion chromatography studies show that in 20 mM potassium phosphate ( pH 7 ) buffer ( KP ) TET4 is approximately twice the length of the form obtained in 20 mM sodium phosphate ( pH 7 ) buffer ( NaP ) and that mixtures of Na + and K + produce mixtures of the two forms whose populations depend on the ratio of the cations .
	manualset3
114621	14	403441	5	NULL	NULL	0	NULL	mixtures 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR semiselective spin-lattice relaxation rate measurements and HPLC size-exclusion chromatography studies show that in 20 mM potassium phosphate ( pH 7 ) buffer ( KP ) TET4 is approximately twice the length of the form obtained in 20 mM sodium phosphate ( pH 7 ) buffer ( NaP ) and that mixtures of Na + and K + produce mixtures of the two forms whose populations depend on the ratio of the cations .
	manualset3
114622	15	403441	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR semiselective spin-lattice relaxation rate measurements and HPLC size-exclusion chromatography studies show that in 20 mM potassium phosphate ( pH 7 ) buffer ( KP ) TET4 is approximately twice the length of the form obtained in 20 mM sodium phosphate ( pH 7 ) buffer ( NaP ) and that mixtures of Na + and K + produce mixtures of the two forms whose populations depend on the ratio of the cations .
	manualset3
114623	16	403441	5	NULL	NULL	0	NULL	forms 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR semiselective spin-lattice relaxation rate measurements and HPLC size-exclusion chromatography studies show that in 20 mM potassium phosphate ( pH 7 ) buffer ( KP ) TET4 is approximately twice the length of the form obtained in 20 mM sodium phosphate ( pH 7 ) buffer ( NaP ) and that mixtures of Na + and K + produce mixtures of the two forms whose populations depend on the ratio of the cations .
	manualset3
114624	17	403441	5	NULL	NULL	0	NULL	populations 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR semiselective spin-lattice relaxation rate measurements and HPLC size-exclusion chromatography studies show that in 20 mM potassium phosphate ( pH 7 ) buffer ( KP ) TET4 is approximately twice the length of the form obtained in 20 mM sodium phosphate ( pH 7 ) buffer ( NaP ) and that mixtures of Na + and K + produce mixtures of the two forms whose populations depend on the ratio of the cations .
	manualset3
114625	18	403441	5	NULL	NULL	0	NULL	ratio 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR semiselective spin-lattice relaxation rate measurements and HPLC size-exclusion chromatography studies show that in 20 mM potassium phosphate ( pH 7 ) buffer ( KP ) TET4 is approximately twice the length of the form obtained in 20 mM sodium phosphate ( pH 7 ) buffer ( NaP ) and that mixtures of Na + and K + produce mixtures of the two forms whose populations depend on the ratio of the cations .
	manualset3
114626	19	403441	5	NULL	NULL	0	NULL	cations 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR semiselective spin-lattice relaxation rate measurements and HPLC size-exclusion chromatography studies show that in 20 mM potassium phosphate ( pH 7 ) buffer ( KP ) TET4 is approximately twice the length of the form obtained in 20 mM sodium phosphate ( pH 7 ) buffer ( NaP ) and that mixtures of Na + and K + produce mixtures of the two forms whose populations depend on the ratio of the cations .
	manualset3
114627	1	403442	5	NULL	NULL	0	NULL	NO 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	NO and its derivatives are also involved in the pathogenic processes in various types of diseases including , but not limited to , neurodegenerative disorders .
	manualset3
114628	2	403442	5	NULL	NULL	0	NULL	derivatives 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	NO and its derivatives are also involved in the pathogenic processes in various types of diseases including , but not limited to , neurodegenerative disorders .
	manualset3
114629	3	403442	5	NULL	NULL	0	NULL	pathogenic processes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	NO and its derivatives are also involved in the pathogenic processes in various types of diseases including , but not limited to , neurodegenerative disorders .
	manualset3
114630	4	403442	5	NULL	NULL	0	NULL	various types	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	NO and its derivatives are also involved in the pathogenic processes in various types of diseases including , but not limited to , neurodegenerative disorders .
	manualset3
114631	5	403442	5	NULL	NULL	0	NULL	diseases 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	NO and its derivatives are also involved in the pathogenic processes in various types of diseases including , but not limited to , neurodegenerative disorders .
	manualset3
114632	6	403442	5	NULL	NULL	0	NULL	neurodegenerative disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	NO and its derivatives are also involved in the pathogenic processes in various types of diseases including , but not limited to , neurodegenerative disorders .
	manualset3
114633	1	403443	5	NULL	NULL	0	NULL	NO application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	NO application and the cue1/nox1 mutation caused decreased PIN-FORMED 1 ( PIN1 ) - GFP fluorescence in a proteasome-independent manner .
	manualset3
114634	2	403443	5	NULL	NULL	0	NULL	cue1/nox1 mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	NO application and the cue1/nox1 mutation caused decreased PIN-FORMED 1 ( PIN1 ) - GFP fluorescence in a proteasome-independent manner .
	manualset3
114635	3	403443	5	NULL	NULL	0	NULL	 PIN-FORMED 1 ( PIN1 ) - GFP fluorescence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	NO application and the cue1/nox1 mutation caused decreased PIN-FORMED 1 ( PIN1 ) - GFP fluorescence in a proteasome-independent manner .
	manualset3
114636	4	403443	5	NULL	NULL	0	NULL	proteasome-independent manner	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	NO application and the cue1/nox1 mutation caused decreased PIN-FORMED 1 ( PIN1 ) - GFP fluorescence in a proteasome-independent manner .
	manualset3
114637	1	403444	5	NULL	NULL	0	NULL	communication situation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A communication situation is described in which the rewards of both members of a pair of monkeys can not exceed chance levels unless the operator monkey responds to cues provided by the informant monkey which indicate the location of food .
	manualset3
114638	2	403444	5	NULL	NULL	0	NULL	rewards 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A communication situation is described in which the rewards of both members of a pair of monkeys can not exceed chance levels unless the operator monkey responds to cues provided by the informant monkey which indicate the location of food .
	manualset3
114639	3	403444	5	NULL	NULL	NULL	NULL	both members	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A communication situation is described in which the rewards of both members of a pair of monkeys can not exceed chance levels unless the operator monkey responds to cues provided by the informant monkey which indicate the location of food .
	manualset3
114640	4	403444	5	NULL	NULL	0	NULL	pair 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A communication situation is described in which the rewards of both members of a pair of monkeys can not exceed chance levels unless the operator monkey responds to cues provided by the informant monkey which indicate the location of food .
	manualset3
114641	5	403444	5	NULL	NULL	0	NULL	monkeys 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A communication situation is described in which the rewards of both members of a pair of monkeys can not exceed chance levels unless the operator monkey responds to cues provided by the informant monkey which indicate the location of food .
	manualset3
114642	6	403444	5	NULL	NULL	0	NULL	chance levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A communication situation is described in which the rewards of both members of a pair of monkeys can not exceed chance levels unless the operator monkey responds to cues provided by the informant monkey which indicate the location of food .
	manualset3
114643	7	403444	5	NULL	NULL	0	NULL	operator monkey 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A communication situation is described in which the rewards of both members of a pair of monkeys can not exceed chance levels unless the operator monkey responds to cues provided by the informant monkey which indicate the location of food .
	manualset3
114644	8	403444	5	NULL	NULL	0	NULL	cues 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A communication situation is described in which the rewards of both members of a pair of monkeys can not exceed chance levels unless the operator monkey responds to cues provided by the informant monkey which indicate the location of food .
	manualset3
114645	9	403444	5	NULL	NULL	0	NULL	informant monkey	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A communication situation is described in which the rewards of both members of a pair of monkeys can not exceed chance levels unless the operator monkey responds to cues provided by the informant monkey which indicate the location of food .
	manualset3
114646	10	403444	5	NULL	NULL	0	NULL	location 	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A communication situation is described in which the rewards of both members of a pair of monkeys can not exceed chance levels unless the operator monkey responds to cues provided by the informant monkey which indicate the location of food .
	manualset3
114647	11	403444	5	NULL	NULL	0	NULL	food 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A communication situation is described in which the rewards of both members of a pair of monkeys can not exceed chance levels unless the operator monkey responds to cues provided by the informant monkey which indicate the location of food .
	manualset3
114648	1	403445	5	NULL	NULL	0	NULL	NO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	NO may also directly S-nitrosylate cysteine residues of specific proteins .
	manualset3
114649	2	403445	5	NULL	NULL	0	NULL	S-nitrosylate cysteine residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	NO may also directly S-nitrosylate cysteine residues of specific proteins .
	manualset3
114650	3	403445	5	NULL	NULL	0	NULL	specific proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	NO may also directly S-nitrosylate cysteine residues of specific proteins .
	manualset3
114651	1	403446	5	NULL	NULL	0	NULL	NPM-ALK	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	NPM-ALK Reverse Transcriptase-Polymerase Chain Reaction Analysis for Detection of the t ( 2 ; 5 ) Translocation of Non-Hodgkin 's Lymphoma .
	manualset3
114652	2	403446	5	NULL	NULL	0	NULL	Reverse Transcriptase-Polymerase Chain Reaction Analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	NPM-ALK Reverse Transcriptase-Polymerase Chain Reaction Analysis for Detection of the t ( 2 ; 5 ) Translocation of Non-Hodgkin 's Lymphoma .
	manualset3
114653	3	403446	5	NULL	NULL	0	NULL	Detection 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	NPM-ALK Reverse Transcriptase-Polymerase Chain Reaction Analysis for Detection of the t ( 2 ; 5 ) Translocation of Non-Hodgkin 's Lymphoma .
	manualset3
114654	4	403446	5	NULL	NULL	0	NULL	t ( 2 ; 5 ) Translocation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	NPM-ALK Reverse Transcriptase-Polymerase Chain Reaction Analysis for Detection of the t ( 2 ; 5 ) Translocation of Non-Hodgkin 's Lymphoma .
	manualset3
114655	5	403446	5	NULL	NULL	0	NULL	Non-Hodgkin 's Lymphoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	NPM-ALK Reverse Transcriptase-Polymerase Chain Reaction Analysis for Detection of the t ( 2 ; 5 ) Translocation of Non-Hodgkin 's Lymphoma .
	manualset3
114656	1	403447	5	NULL	NULL	0	NULL	NPY-IR	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	NPY-IR was transiently expressed in the granule cells/mossy fibers after the preconvulsive stage 2 and 2 days but not 1 week after three consecutive tonic-clonic seizures ( stage 5 ) .
	manualset3
114657	2	403447	5	NULL	NULL	0	NULL	granule cells/mossy fibers	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	NPY-IR was transiently expressed in the granule cells/mossy fibers after the preconvulsive stage 2 and 2 days but not 1 week after three consecutive tonic-clonic seizures ( stage 5 ) .
	manualset3
114658	3	403447	5	NULL	NULL	0	NULL	preconvulsive stage 2	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	NPY-IR was transiently expressed in the granule cells/mossy fibers after the preconvulsive stage 2 and 2 days but not 1 week after three consecutive tonic-clonic seizures ( stage 5 ) .
	manualset3
114659	4	403447	5	NULL	NULL	0	NULL	2 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	NPY-IR was transiently expressed in the granule cells/mossy fibers after the preconvulsive stage 2 and 2 days but not 1 week after three consecutive tonic-clonic seizures ( stage 5 ) .
	manualset3
114660	5	403447	5	NULL	NULL	0	NULL	1 week 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	NPY-IR was transiently expressed in the granule cells/mossy fibers after the preconvulsive stage 2 and 2 days but not 1 week after three consecutive tonic-clonic seizures ( stage 5 ) .
	manualset3
114661	6	403447	5	NULL	NULL	0	NULL	three consecutive tonic-clonic seizures ( stage 5 )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	NPY-IR was transiently expressed in the granule cells/mossy fibers after the preconvulsive stage 2 and 2 days but not 1 week after three consecutive tonic-clonic seizures ( stage 5 ) .
	manualset3
114662	1	403448	5	NULL	NULL	0	NULL	NPY 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	NPY had no effect on basal steroid release from the Y-1 cells .
	manualset3
114663	2	403448	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	NPY had no effect on basal steroid release from the Y-1 cells .
	manualset3
114664	3	403448	5	NULL	NULL	0	NULL	basal steroid release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	NPY had no effect on basal steroid release from the Y-1 cells .
	manualset3
114665	4	403448	5	NULL	NULL	0	NULL	Y-1 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	NPY had no effect on basal steroid release from the Y-1 cells .
	manualset3
114666	1	403449	5	NULL	NULL	0	NULL	NQO1 mRNA levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	NQO1 mRNA levels and NQO1 DNA polymorphism analysis indicated different underlying mechanisms : reduced expression and selection of the inactive NQO1 * 2 polymorphism .
	manualset3
114667	2	403449	5	NULL	NULL	0	NULL	NQO1 DNA polymorphism analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	NQO1 mRNA levels and NQO1 DNA polymorphism analysis indicated different underlying mechanisms : reduced expression and selection of the inactive NQO1 * 2 polymorphism .
	manualset3
114668	3	403449	5	NULL	NULL	0	NULL	underlying mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	NQO1 mRNA levels and NQO1 DNA polymorphism analysis indicated different underlying mechanisms : reduced expression and selection of the inactive NQO1 * 2 polymorphism .
	manualset3
114669	4	403449	5	NULL	NULL	0	NULL	reduced expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	NQO1 mRNA levels and NQO1 DNA polymorphism analysis indicated different underlying mechanisms : reduced expression and selection of the inactive NQO1 * 2 polymorphism .
	manualset3
114670	5	403449	5	NULL	NULL	0	NULL	selection 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	NQO1 mRNA levels and NQO1 DNA polymorphism analysis indicated different underlying mechanisms : reduced expression and selection of the inactive NQO1 * 2 polymorphism .
	manualset3
114671	6	403449	5	NULL	NULL	0	NULL	inactive NQO1 * 2 polymorphism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	NQO1 mRNA levels and NQO1 DNA polymorphism analysis indicated different underlying mechanisms : reduced expression and selection of the inactive NQO1 * 2 polymorphism .
	manualset3
114672	1	403450	5	NULL	NULL	0	NULL	NR2B-NMDA receptor-mediated increases in intracellular Ca2 + concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	NR2B-NMDA receptor-mediated increases in intracellular Ca2 + concentration regulate the tyrosine phosphatase , STEP , and ERK MAP kinase signaling .
	manualset3
114673	2	403450	5	NULL	NULL	0	NULL	tyrosine phosphatase signaling 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	NR2B-NMDA receptor-mediated increases in intracellular Ca2 + concentration regulate the tyrosine phosphatase , STEP , and ERK MAP kinase signaling .
	manualset3
114674	3	403450	5	NULL	NULL	0	NULL	STEP signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	NR2B-NMDA receptor-mediated increases in intracellular Ca2 + concentration regulate the tyrosine phosphatase , STEP , and ERK MAP kinase signaling .
	manualset3
114675	4	403450	5	NULL	NULL	0	NULL	ERK MAP kinase signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	NR2B-NMDA receptor-mediated increases in intracellular Ca2 + concentration regulate the tyrosine phosphatase , STEP , and ERK MAP kinase signaling .
	manualset3
114724	1	403451	5	NULL	NULL	0	NULL	NSAIDs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	NSAIDs have demonstrated efficacy superior to placebo in patients with osteoarthritis .
	manualset3
114725	2	403451	5	NULL	NULL	0	NULL	efficacy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	NSAIDs have demonstrated efficacy superior to placebo in patients with osteoarthritis .
	manualset3
114727	3	403451	5	NULL	NULL	0	NULL	placebo	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	NSAIDs have demonstrated efficacy superior to placebo in patients with osteoarthritis .
	manualset3
114728	4	403451	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	NSAIDs have demonstrated efficacy superior to placebo in patients with osteoarthritis .
	manualset3
114729	5	403451	5	NULL	NULL	0	NULL	osteoarthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	NSAIDs have demonstrated efficacy superior to placebo in patients with osteoarthritis .
	manualset3
114737	1	403452	5	NULL	NULL	0	NULL	NSF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	NSF was found to be present in the cytosol of rat pancreatic beta-cells and rat insulinoma INS-1 cells .
	manualset3
114738	2	403452	5	NULL	NULL	0	NULL	cytosol	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	NSF was found to be present in the cytosol of rat pancreatic beta-cells and rat insulinoma INS-1 cells .
	manualset3
114741	3	403452	5	NULL	NULL	0	NULL	rat pancreatic beta-cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	NSF was found to be present in the cytosol of rat pancreatic beta-cells and rat insulinoma INS-1 cells .
	manualset3
114743	4	403452	5	NULL	NULL	0	NULL	rat insulinoma INS-1 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	NSF was found to be present in the cytosol of rat pancreatic beta-cells and rat insulinoma INS-1 cells .
	manualset3
114748	1	403453	5	NULL	NULL	0	NULL	NSP4-positive cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	NSP4-positive cells had strongly positive expression of integrin subunit 2 .
	manualset3
114750	2	403453	5	NULL	NULL	0	NULL	strongly positive expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	NSP4-positive cells had strongly positive expression of integrin subunit 2 .
	manualset3
114751	3	403453	5	NULL	NULL	0	NULL	integrin subunit 2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	NSP4-positive cells had strongly positive expression of integrin subunit 2 .
	manualset3
114884	1	403454	5	NULL	NULL	0	NULL	NV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	NV , HAV , and FCV were inoculated into marinated mussels and marinade liquid and then held at 4 degrees C for up to 4 weeks .
	manualset3
114885	2	403454	5	NULL	NULL	0	NULL	HAV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	NV , HAV , and FCV were inoculated into marinated mussels and marinade liquid and then held at 4 degrees C for up to 4 weeks .
	manualset3
114886	3	403454	5	NULL	NULL	0	NULL	FCV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	NV , HAV , and FCV were inoculated into marinated mussels and marinade liquid and then held at 4 degrees C for up to 4 weeks .
	manualset3
114887	4	403454	5	NULL	NULL	0	NULL	marinated mussels	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	NV , HAV , and FCV were inoculated into marinated mussels and marinade liquid and then held at 4 degrees C for up to 4 weeks .
	manualset3
114888	5	403454	5	NULL	NULL	0	NULL	marinade liquid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	NV , HAV , and FCV were inoculated into marinated mussels and marinade liquid and then held at 4 degrees C for up to 4 weeks .
	manualset3
114889	6	403454	5	NULL	NULL	0	NULL	4 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	NV , HAV , and FCV were inoculated into marinated mussels and marinade liquid and then held at 4 degrees C for up to 4 weeks .
	manualset3
114890	7	403454	5	NULL	NULL	0	NULL	4 weeks	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	NV , HAV , and FCV were inoculated into marinated mussels and marinade liquid and then held at 4 degrees C for up to 4 weeks .
	manualset3
114891	1	403455	5	NULL	NULL	NULL	NULL	Na , K-ATPase alpha subunit gene	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Na , K-ATPase alpha and beta subunit genes exhibit unique expression patterns during zebrafish embryogenesis .
	manualset3
114892	2	403455	5	NULL	NULL	0	NULL	Na , K-ATPase beta subunit gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Na , K-ATPase alpha and beta subunit genes exhibit unique expression patterns during zebrafish embryogenesis .
	manualset3
114893	3	403455	5	NULL	NULL	0	NULL	unique expression patterns	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Na , K-ATPase alpha and beta subunit genes exhibit unique expression patterns during zebrafish embryogenesis .
	manualset3
114894	4	403455	5	NULL	NULL	0	NULL	zebrafish embryogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Na , K-ATPase alpha and beta subunit genes exhibit unique expression patterns during zebrafish embryogenesis .
	manualset3
114895	1	403456	5	NULL	NULL	0	NULL	Na/Ca exchange	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Na/Ca exchange is assumed to be of minor importance and the Na/H exchange may be involved .
	manualset3
114896	2	403456	5	NULL	NULL	0	NULL	minor importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Na/Ca exchange is assumed to be of minor importance and the Na/H exchange may be involved .
	manualset3
114897	3	403456	5	NULL	NULL	0	NULL	Na/H exchange 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Na/Ca exchange is assumed to be of minor importance and the Na/H exchange may be involved .
	manualset3
114898	1	403457	5	NULL	NULL	0	NULL	Nalbuphine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Nalbuphine and pentazocine in an opioid-benzodiazepine sedative technique : a double-blind comparison .
	manualset3
114899	2	403457	5	NULL	NULL	0	NULL	pentazocine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Nalbuphine and pentazocine in an opioid-benzodiazepine sedative technique : a double-blind comparison .
	manualset3
114900	3	403457	5	NULL	NULL	0	NULL	opioid-benzodiazepine sedative technique 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Nalbuphine and pentazocine in an opioid-benzodiazepine sedative technique : a double-blind comparison .
	manualset3
114901	4	403457	5	NULL	NULL	0	NULL	double-blind comparison	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nalbuphine and pentazocine in an opioid-benzodiazepine sedative technique : a double-blind comparison .
	manualset3
114902	1	403458	5	NULL	NULL	0	NULL	Naloxone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Naloxone ( 1 mg/kg ) significantly changed the spectrum of ultradian rhythms , but did not alter the length and phase of circadian periodicity .
	manualset3
114903	2	403458	5	NULL	NULL	0	NULL	1 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Naloxone ( 1 mg/kg ) significantly changed the spectrum of ultradian rhythms , but did not alter the length and phase of circadian periodicity .
	manualset3
114904	3	403458	5	NULL	NULL	0	NULL	spectrum	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Naloxone ( 1 mg/kg ) significantly changed the spectrum of ultradian rhythms , but did not alter the length and phase of circadian periodicity .
	manualset3
114905	4	403458	5	NULL	NULL	0	NULL	ultradian rhythms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Naloxone ( 1 mg/kg ) significantly changed the spectrum of ultradian rhythms , but did not alter the length and phase of circadian periodicity .
	manualset3
114906	5	403458	5	NULL	NULL	0	NULL	length	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Naloxone ( 1 mg/kg ) significantly changed the spectrum of ultradian rhythms , but did not alter the length and phase of circadian periodicity .
	manualset3
114907	6	403458	5	NULL	NULL	0	NULL	phase	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Naloxone ( 1 mg/kg ) significantly changed the spectrum of ultradian rhythms , but did not alter the length and phase of circadian periodicity .
	manualset3
114908	7	403458	5	NULL	NULL	0	NULL	circadian periodicity	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Naloxone ( 1 mg/kg ) significantly changed the spectrum of ultradian rhythms , but did not alter the length and phase of circadian periodicity .
	manualset3
114909	1	403459	5	NULL	NULL	0	NULL	Naltrexone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Naltrexone antagonized the inhibitory effect of morphine on IFN-alpha expression in NT2-N cells .
	manualset3
114910	2	403459	5	NULL	NULL	0	NULL	inhibitory effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Naltrexone antagonized the inhibitory effect of morphine on IFN-alpha expression in NT2-N cells .
	manualset3
114911	3	403459	5	NULL	NULL	0	NULL	morphine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Naltrexone antagonized the inhibitory effect of morphine on IFN-alpha expression in NT2-N cells .
	manualset3
114912	4	403459	5	NULL	NULL	0	NULL	IFN-alpha expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Naltrexone antagonized the inhibitory effect of morphine on IFN-alpha expression in NT2-N cells .
	manualset3
114913	5	403459	5	NULL	NULL	0	NULL	NT2-N cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Naltrexone antagonized the inhibitory effect of morphine on IFN-alpha expression in NT2-N cells .
	manualset3
114914	1	403460	5	NULL	NULL	0	NULL	Naltrexone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Naltrexone did not effect PAG induced suppression of peripheral blood NK .
	manualset3
114915	2	403460	5	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Naltrexone did not effect PAG induced suppression of peripheral blood NK .
	manualset3
114916	3	403460	5	NULL	NULL	0	NULL	PAG induced suppression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Naltrexone did not effect PAG induced suppression of peripheral blood NK .
	manualset3
114917	4	403460	5	NULL	NULL	0	NULL	peripheral blood NK	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Naltrexone did not effect PAG induced suppression of peripheral blood NK .
	manualset3
114918	1	403461	5	NULL	NULL	0	NULL	BMP-15	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Namely , BMP-15 stimulates granulosa cell mitosis and inhibits follicle-stimulating hormone ( FSH ) receptor mRNA expression in granulosa cell , thereby playing a critical role in the elaborate mechanism controlling ovarian folliculogenesis .
	manualset3
114919	2	403461	5	NULL	NULL	0	NULL	granulosa cell mitosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Namely , BMP-15 stimulates granulosa cell mitosis and inhibits follicle-stimulating hormone ( FSH ) receptor mRNA expression in granulosa cell , thereby playing a critical role in the elaborate mechanism controlling ovarian folliculogenesis .
	manualset3
114920	3	403461	5	NULL	NULL	0	NULL	follicle-stimulating hormone ( FSH ) receptor mRNA expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Namely , BMP-15 stimulates granulosa cell mitosis and inhibits follicle-stimulating hormone ( FSH ) receptor mRNA expression in granulosa cell , thereby playing a critical role in the elaborate mechanism controlling ovarian folliculogenesis .
	manualset3
114921	4	403461	5	NULL	NULL	0	NULL	granulosa cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Namely , BMP-15 stimulates granulosa cell mitosis and inhibits follicle-stimulating hormone ( FSH ) receptor mRNA expression in granulosa cell , thereby playing a critical role in the elaborate mechanism controlling ovarian folliculogenesis .
	manualset3
114922	5	403461	5	NULL	NULL	0	NULL	critical role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Namely , BMP-15 stimulates granulosa cell mitosis and inhibits follicle-stimulating hormone ( FSH ) receptor mRNA expression in granulosa cell , thereby playing a critical role in the elaborate mechanism controlling ovarian folliculogenesis .
	manualset3
114923	6	403461	5	NULL	NULL	0	NULL	mechanism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Namely , BMP-15 stimulates granulosa cell mitosis and inhibits follicle-stimulating hormone ( FSH ) receptor mRNA expression in granulosa cell , thereby playing a critical role in the elaborate mechanism controlling ovarian folliculogenesis .
	manualset3
114924	7	403461	5	NULL	NULL	0	NULL	ovarian folliculogenesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Namely , BMP-15 stimulates granulosa cell mitosis and inhibits follicle-stimulating hormone ( FSH ) receptor mRNA expression in granulosa cell , thereby playing a critical role in the elaborate mechanism controlling ovarian folliculogenesis .
	manualset3
114925	1	403462	5	NULL	NULL	0	NULL	skill	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Namely , after a skill or memory is acquired , it must be consolidated before it becomes resistant to disruption by subsequent learning .
	manualset3
114926	2	403462	5	NULL	NULL	0	NULL	memory	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Namely , after a skill or memory is acquired , it must be consolidated before it becomes resistant to disruption by subsequent learning .
	manualset3
114927	3	403462	5	NULL	NULL	0	NULL	disruption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Namely , after a skill or memory is acquired , it must be consolidated before it becomes resistant to disruption by subsequent learning .
	manualset3
114928	4	403462	5	NULL	NULL	0	NULL	subsequent learning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Namely , after a skill or memory is acquired , it must be consolidated before it becomes resistant to disruption by subsequent learning .
	manualset3
114929	1	403463	5	NULL	NULL	0	NULL	Nano-composites	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nano-composites are manufactured from pure quartzose sand .
	manualset3
114930	2	403463	5	NULL	NULL	NULL	NULL	pure quartzose sand	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nano-composites are manufactured from pure quartzose sand .
	manualset3
114931	1	403464	5	NULL	NULL	0	NULL	Nanocomposite formulation system	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanocomposite formulation system of lipid-regulating drugs based on layered double hydroxide : synthesis , characterization and drug release properties .
	manualset3
114932	2	403464	5	NULL	NULL	0	NULL	lipid-regulating drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanocomposite formulation system of lipid-regulating drugs based on layered double hydroxide : synthesis , characterization and drug release properties .
	manualset3
115023	3	403464	5	NULL	NULL	0	NULL	layered double hydroxide	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanocomposite formulation system of lipid-regulating drugs based on layered double hydroxide : synthesis , characterization and drug release properties .
	manualset3
115024	4	403464	5	NULL	NULL	0	NULL	synthesis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanocomposite formulation system of lipid-regulating drugs based on layered double hydroxide : synthesis , characterization and drug release properties .
	manualset3
115025	5	403464	5	NULL	NULL	0	NULL	characterization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanocomposite formulation system of lipid-regulating drugs based on layered double hydroxide : synthesis , characterization and drug release properties .
	manualset3
115026	6	403464	5	NULL	NULL	0	NULL	drug release properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanocomposite formulation system of lipid-regulating drugs based on layered double hydroxide : synthesis , characterization and drug release properties .
	manualset3
115044	1	403465	5	NULL	NULL	0	NULL	Nanofiltration ( NF ) experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanofiltration ( NF ) experiments were conducted with simulated solution containing bicarbonate hardness and with three membranes : NF90 , NF270 and NF - .
	manualset3
115045	2	403465	5	NULL	NULL	0	NULL	simulated solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanofiltration ( NF ) experiments were conducted with simulated solution containing bicarbonate hardness and with three membranes : NF90 , NF270 and NF - .
	manualset3
115046	3	403465	5	NULL	NULL	0	NULL	bicarbonate hardness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanofiltration ( NF ) experiments were conducted with simulated solution containing bicarbonate hardness and with three membranes : NF90 , NF270 and NF - .
	manualset3
115047	4	403465	5	NULL	NULL	0	NULL	three	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanofiltration ( NF ) experiments were conducted with simulated solution containing bicarbonate hardness and with three membranes : NF90 , NF270 and NF - .
	manualset3
115048	5	403465	5	NULL	NULL	0	NULL	membranes	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanofiltration ( NF ) experiments were conducted with simulated solution containing bicarbonate hardness and with three membranes : NF90 , NF270 and NF - .
	manualset3
115056	6	403465	5	NULL	NULL	0	NULL	NF90 membrane	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanofiltration ( NF ) experiments were conducted with simulated solution containing bicarbonate hardness and with three membranes : NF90 , NF270 and NF - .
	manualset3
115057	7	403465	5	NULL	NULL	0	NULL	NF270 membrane	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanofiltration ( NF ) experiments were conducted with simulated solution containing bicarbonate hardness and with three membranes : NF90 , NF270 and NF - .
	manualset3
115058	8	403465	5	NULL	NULL	0	NULL	NF membrane	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanofiltration ( NF ) experiments were conducted with simulated solution containing bicarbonate hardness and with three membranes : NF90 , NF270 and NF - .
	manualset3
115059	1	403466	5	NULL	NULL	0	NULL	Nanog	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanog , a key transcription factor in self-renewal and pluripotency of embryonic stem cells , has been proved to play a novel role in solid tumor development .
	manualset3
115060	2	403466	5	NULL	NULL	0	NULL	key transcription factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanog , a key transcription factor in self-renewal and pluripotency of embryonic stem cells , has been proved to play a novel role in solid tumor development .
	manualset3
115061	3	403466	5	NULL	NULL	0	NULL	self-renewal	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanog , a key transcription factor in self-renewal and pluripotency of embryonic stem cells , has been proved to play a novel role in solid tumor development .
	manualset3
115062	4	403466	5	NULL	NULL	0	NULL	pluripotency	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanog , a key transcription factor in self-renewal and pluripotency of embryonic stem cells , has been proved to play a novel role in solid tumor development .
	manualset3
115063	5	403466	5	NULL	NULL	0	NULL	embryonic stem cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanog , a key transcription factor in self-renewal and pluripotency of embryonic stem cells , has been proved to play a novel role in solid tumor development .
	manualset3
115064	6	403466	5	NULL	NULL	0	NULL	novel role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanog , a key transcription factor in self-renewal and pluripotency of embryonic stem cells , has been proved to play a novel role in solid tumor development .
	manualset3
115065	7	403466	5	NULL	NULL	0	NULL	solid tumor development	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanog , a key transcription factor in self-renewal and pluripotency of embryonic stem cells , has been proved to play a novel role in solid tumor development .
	manualset3
115066	1	403467	5	NULL	NULL	0	NULL	Nanopipette delivery	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanopipette delivery of individual molecules to cellular compartments for single-molecule fluorescence tracking .
	manualset3
115067	2	403467	5	NULL	NULL	0	NULL	individual molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanopipette delivery of individual molecules to cellular compartments for single-molecule fluorescence tracking .
	manualset3
115068	3	403467	5	NULL	NULL	0	NULL	cellular compartments	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanopipette delivery of individual molecules to cellular compartments for single-molecule fluorescence tracking .
	manualset3
115069	4	403467	5	NULL	NULL	0	NULL	single-molecule fluorescence tracking	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanopipette delivery of individual molecules to cellular compartments for single-molecule fluorescence tracking .
	manualset3
115070	1	403468	5	NULL	NULL	0	NULL	Nanosecond motions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanosecond motions of the single tryptophan residues in apolipoproteins C-I and C-II : a study by oxygen quenching and fluorescence depolarization .
	manualset3
115071	2	403468	5	NULL	NULL	0	NULL	single tryptophan residues 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanosecond motions of the single tryptophan residues in apolipoproteins C-I and C-II : a study by oxygen quenching and fluorescence depolarization .
	manualset3
115072	3	403468	5	NULL	NULL	0	NULL	apolipoprotein C-I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanosecond motions of the single tryptophan residues in apolipoproteins C-I and C-II : a study by oxygen quenching and fluorescence depolarization .
	manualset3
115073	4	403468	5	NULL	NULL	0	NULL	apolipoprotein C-II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanosecond motions of the single tryptophan residues in apolipoproteins C-I and C-II : a study by oxygen quenching and fluorescence depolarization .
	manualset3
115074	5	403468	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanosecond motions of the single tryptophan residues in apolipoproteins C-I and C-II : a study by oxygen quenching and fluorescence depolarization .
	manualset3
115075	6	403468	5	NULL	NULL	0	NULL	oxygen quenching	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanosecond motions of the single tryptophan residues in apolipoproteins C-I and C-II : a study by oxygen quenching and fluorescence depolarization .
	manualset3
115076	7	403468	5	NULL	NULL	0	NULL	fluorescence depolarization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nanosecond motions of the single tryptophan residues in apolipoproteins C-I and C-II : a study by oxygen quenching and fluorescence depolarization .
	manualset3
115077	1	403469	5	NULL	NULL	0	NULL	comparative analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative analysis of the results of treatment of two groups of patients with carcinoma of the rectum was made for a 6-year period of observation .
	manualset3
115078	2	403469	5	NULL	NULL	0	NULL	results 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative analysis of the results of treatment of two groups of patients with carcinoma of the rectum was made for a 6-year period of observation .
	manualset3
115079	3	403469	5	NULL	NULL	0	NULL	treatment 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative analysis of the results of treatment of two groups of patients with carcinoma of the rectum was made for a 6-year period of observation .
	manualset3
115080	4	403469	5	NULL	NULL	0	NULL	two groups	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative analysis of the results of treatment of two groups of patients with carcinoma of the rectum was made for a 6-year period of observation .
	manualset3
115081	5	403469	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative analysis of the results of treatment of two groups of patients with carcinoma of the rectum was made for a 6-year period of observation .
	manualset3
115082	6	403469	5	NULL	NULL	0	NULL	carcinoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative analysis of the results of treatment of two groups of patients with carcinoma of the rectum was made for a 6-year period of observation .
	manualset3
115083	7	403469	5	NULL	NULL	0	NULL	rectum 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative analysis of the results of treatment of two groups of patients with carcinoma of the rectum was made for a 6-year period of observation .
	manualset3
115084	8	403469	5	NULL	NULL	0	NULL	6-year period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative analysis of the results of treatment of two groups of patients with carcinoma of the rectum was made for a 6-year period of observation .
	manualset3
115085	9	403469	5	NULL	NULL	0	NULL	observation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative analysis of the results of treatment of two groups of patients with carcinoma of the rectum was made for a 6-year period of observation .
	manualset3
115086	1	403470	5	NULL	NULL	0	NULL	Naphthomycin K	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Naphthomycin K showed evident cytotoxicity against P388 and A-549 cell lines , but no inhibitory activities against Staphylococcus aureus and Mycobacterium tuberculosis .
	manualset3
115087	2	403470	5	NULL	NULL	0	NULL	cytotoxicity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Naphthomycin K showed evident cytotoxicity against P388 and A-549 cell lines , but no inhibitory activities against Staphylococcus aureus and Mycobacterium tuberculosis .
	manualset3
115088	3	403470	5	NULL	NULL	0	NULL	P388 cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Naphthomycin K showed evident cytotoxicity against P388 and A-549 cell lines , but no inhibitory activities against Staphylococcus aureus and Mycobacterium tuberculosis .
	manualset3
115089	4	403470	5	NULL	NULL	0	NULL	A-549 cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Naphthomycin K showed evident cytotoxicity against P388 and A-549 cell lines , but no inhibitory activities against Staphylococcus aureus and Mycobacterium tuberculosis .
	manualset3
115090	5	403470	5	NULL	NULL	0	NULL	inhibitory activities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Naphthomycin K showed evident cytotoxicity against P388 and A-549 cell lines , but no inhibitory activities against Staphylococcus aureus and Mycobacterium tuberculosis .
	manualset3
115091	6	403470	5	NULL	NULL	0	NULL	Staphylococcus aureus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Naphthomycin K showed evident cytotoxicity against P388 and A-549 cell lines , but no inhibitory activities against Staphylococcus aureus and Mycobacterium tuberculosis .
	manualset3
115092	7	403470	5	NULL	NULL	0	NULL	Mycobacterium tuberculosis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Naphthomycin K showed evident cytotoxicity against P388 and A-549 cell lines , but no inhibitory activities against Staphylococcus aureus and Mycobacterium tuberculosis .
	manualset3
115093	1	403471	5	NULL	NULL	0	NULL	Naproxen release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Naproxen release from sustained release matrix system and effect of cellulose derivatives .
	manualset3
115094	2	403471	5	NULL	NULL	0	NULL	release matrix system	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Naproxen release from sustained release matrix system and effect of cellulose derivatives .
	manualset3
115095	3	403471	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Naproxen release from sustained release matrix system and effect of cellulose derivatives .
	manualset3
115096	4	403471	5	NULL	NULL	0	NULL	cellulose derivatives	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Naproxen release from sustained release matrix system and effect of cellulose derivatives .
	manualset3
115097	1	403472	5	NULL	NULL	0	NULL	Narrative skill	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Narrative skill and syntactic complexity in school-age children with and without late language emergence .
	manualset3
115098	2	403472	5	NULL	NULL	0	NULL	syntactic complexity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Narrative skill and syntactic complexity in school-age children with and without late language emergence .
	manualset3
115099	3	403472	5	NULL	NULL	0	NULL	school-age children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Narrative skill and syntactic complexity in school-age children with and without late language emergence .
	manualset3
115100	4	403472	5	NULL	NULL	0	NULL	late language emergence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Narrative skill and syntactic complexity in school-age children with and without late language emergence .
	manualset3
115101	1	403473	5	NULL	NULL	0	NULL	Nasal nitric oxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nasal nitric oxide and regulation of human pulmonary blood flow in the upright position .
	manualset3
115102	2	403473	5	NULL	NULL	0	NULL	regulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nasal nitric oxide and regulation of human pulmonary blood flow in the upright position .
	manualset3
115103	3	403473	5	NULL	NULL	NULL	NULL	human pulmonary blood flow	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nasal nitric oxide and regulation of human pulmonary blood flow in the upright position .
	manualset3
115104	4	403473	5	NULL	NULL	0	NULL	upright position	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nasal nitric oxide and regulation of human pulmonary blood flow in the upright position .
	manualset3
115105	1	403474	5	NULL	NULL	0	NULL	Nasal polyp tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Nasal polyp tissue is characterized by its frequent infiltration by large numbers of eosinophils .
	manualset3
115106	2	403474	5	NULL	NULL	0	NULL	frequent infiltration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nasal polyp tissue is characterized by its frequent infiltration by large numbers of eosinophils .
	manualset3
115107	3	403474	5	NULL	NULL	0	NULL	large numbers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nasal polyp tissue is characterized by its frequent infiltration by large numbers of eosinophils .
	manualset3
115108	4	403474	5	NULL	NULL	0	NULL	eosinophils 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Nasal polyp tissue is characterized by its frequent infiltration by large numbers of eosinophils .
	manualset3
115109	1	403475	5	NULL	NULL	0	NULL	National Institute for Program Director Development ( NIPDD )	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	National Institute for Program Director Development ( NIPDD ) : a collaborative pursuit of excellence .
	manualset3
115110	2	403475	5	NULL	NULL	0	NULL	collaborative pursuit 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	National Institute for Program Director Development ( NIPDD ) : a collaborative pursuit of excellence .
	manualset3
115111	3	403475	5	NULL	NULL	0	NULL	excellence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	National Institute for Program Director Development ( NIPDD ) : a collaborative pursuit of excellence .
	manualset3
115112	1	403476	5	NULL	NULL	0	NULL	National and international tendencies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	National and international tendencies to avoid nasal packing after FESS are closed related to the surgical surgery ( atraumatic endoscopic surgery , avoidance of resection of turbinates , meticulose coagulation ) .
	manualset3
115113	2	403476	5	NULL	NULL	0	NULL	nasal packing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	National and international tendencies to avoid nasal packing after FESS are closed related to the surgical surgery ( atraumatic endoscopic surgery , avoidance of resection of turbinates , meticulose coagulation ) .
	manualset3
115114	3	403476	5	NULL	NULL	0	NULL	FESS 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	National and international tendencies to avoid nasal packing after FESS are closed related to the surgical surgery ( atraumatic endoscopic surgery , avoidance of resection of turbinates , meticulose coagulation ) .
	manualset3
115115	4	403476	5	NULL	NULL	0	NULL	surgical surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	National and international tendencies to avoid nasal packing after FESS are closed related to the surgical surgery ( atraumatic endoscopic surgery , avoidance of resection of turbinates , meticulose coagulation ) .
	manualset3
115116	5	403476	5	NULL	NULL	0	NULL	atraumatic endoscopic surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	National and international tendencies to avoid nasal packing after FESS are closed related to the surgical surgery ( atraumatic endoscopic surgery , avoidance of resection of turbinates , meticulose coagulation ) .
	manualset3
115117	6	403476	5	NULL	NULL	0	NULL	avoidance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	National and international tendencies to avoid nasal packing after FESS are closed related to the surgical surgery ( atraumatic endoscopic surgery , avoidance of resection of turbinates , meticulose coagulation ) .
	manualset3
115118	7	403476	5	NULL	NULL	0	NULL	resection 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	National and international tendencies to avoid nasal packing after FESS are closed related to the surgical surgery ( atraumatic endoscopic surgery , avoidance of resection of turbinates , meticulose coagulation ) .
	manualset3
115119	8	403476	5	NULL	NULL	0	NULL	turbinates 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	National and international tendencies to avoid nasal packing after FESS are closed related to the surgical surgery ( atraumatic endoscopic surgery , avoidance of resection of turbinates , meticulose coagulation ) .
	manualset3
115120	9	403476	5	NULL	NULL	0	NULL	meticulose coagulation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	National and international tendencies to avoid nasal packing after FESS are closed related to the surgical surgery ( atraumatic endoscopic surgery , avoidance of resection of turbinates , meticulose coagulation ) .
	manualset3
115121	1	403477	5	NULL	NULL	0	NULL	comparative immunomorphologic study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative immunomorphologic study was carried out on cryostate sections of renal tissue of plaice ( Pleuronectes platessa L. ) and rat , using specific antibodies against the proteins of intermediate filaments -- cytokeratins and vimentin .
	manualset3
115122	2	403477	5	NULL	NULL	0	NULL	cryostate sections	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative immunomorphologic study was carried out on cryostate sections of renal tissue of plaice ( Pleuronectes platessa L. ) and rat , using specific antibodies against the proteins of intermediate filaments -- cytokeratins and vimentin .
	manualset3
115123	3	403477	5	NULL	NULL	0	NULL	renal tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative immunomorphologic study was carried out on cryostate sections of renal tissue of plaice ( Pleuronectes platessa L. ) and rat , using specific antibodies against the proteins of intermediate filaments -- cytokeratins and vimentin .
	manualset3
115124	4	403477	5	NULL	NULL	0	NULL	plaice ( Pleuronectes platessa L. )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative immunomorphologic study was carried out on cryostate sections of renal tissue of plaice ( Pleuronectes platessa L. ) and rat , using specific antibodies against the proteins of intermediate filaments -- cytokeratins and vimentin .
	manualset3
115125	5	403477	5	NULL	NULL	0	NULL	rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative immunomorphologic study was carried out on cryostate sections of renal tissue of plaice ( Pleuronectes platessa L. ) and rat , using specific antibodies against the proteins of intermediate filaments -- cytokeratins and vimentin .
	manualset3
115126	6	403477	5	NULL	NULL	0	NULL	specific antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative immunomorphologic study was carried out on cryostate sections of renal tissue of plaice ( Pleuronectes platessa L. ) and rat , using specific antibodies against the proteins of intermediate filaments -- cytokeratins and vimentin .
	manualset3
115127	7	403477	5	NULL	NULL	0	NULL	proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative immunomorphologic study was carried out on cryostate sections of renal tissue of plaice ( Pleuronectes platessa L. ) and rat , using specific antibodies against the proteins of intermediate filaments -- cytokeratins and vimentin .
	manualset3
115128	8	403477	5	NULL	NULL	0	NULL	intermediate filaments	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative immunomorphologic study was carried out on cryostate sections of renal tissue of plaice ( Pleuronectes platessa L. ) and rat , using specific antibodies against the proteins of intermediate filaments -- cytokeratins and vimentin .
	manualset3
115129	9	403477	5	NULL	NULL	0	NULL	cytokeratins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative immunomorphologic study was carried out on cryostate sections of renal tissue of plaice ( Pleuronectes platessa L. ) and rat , using specific antibodies against the proteins of intermediate filaments -- cytokeratins and vimentin .
	manualset3
115130	10	403477	5	NULL	NULL	0	NULL	vimentin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative immunomorphologic study was carried out on cryostate sections of renal tissue of plaice ( Pleuronectes platessa L. ) and rat , using specific antibodies against the proteins of intermediate filaments -- cytokeratins and vimentin .
	manualset3
115188	1	403478	5	NULL	NULL	0	NULL	National cholesterol-management guidelines	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	National cholesterol-management guidelines call for aggressive therapy .
	manualset3
115189	2	403478	5	NULL	NULL	0	NULL	aggressive therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	National cholesterol-management guidelines call for aggressive therapy .
	manualset3
115193	1	403479	5	NULL	NULL	0	NULL	Nationwide surveys	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nationwide surveys showed that the average detection rate of C. botulinum spores in soil and foods in the northern parts of China was 14.8 % , while it was only 2.5 % in the south .
	manualset3
115194	2	403479	5	NULL	NULL	0	NULL	average detection rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nationwide surveys showed that the average detection rate of C. botulinum spores in soil and foods in the northern parts of China was 14.8 % , while it was only 2.5 % in the south .
	manualset3
115199	3	403479	5	NULL	NULL	0	NULL	C. botulinum spores	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Nationwide surveys showed that the average detection rate of C. botulinum spores in soil and foods in the northern parts of China was 14.8 % , while it was only 2.5 % in the south .
	manualset3
115201	4	403479	5	NULL	NULL	0	NULL	soil	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Nationwide surveys showed that the average detection rate of C. botulinum spores in soil and foods in the northern parts of China was 14.8 % , while it was only 2.5 % in the south .
	manualset3
115202	5	403479	5	NULL	NULL	0	NULL	foods	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Nationwide surveys showed that the average detection rate of C. botulinum spores in soil and foods in the northern parts of China was 14.8 % , while it was only 2.5 % in the south .
	manualset3
115203	6	403479	5	NULL	NULL	0	NULL	northern parts of China	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Nationwide surveys showed that the average detection rate of C. botulinum spores in soil and foods in the northern parts of China was 14.8 % , while it was only 2.5 % in the south .
	manualset3
115204	7	403479	5	NULL	NULL	0	NULL	14.8 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Nationwide surveys showed that the average detection rate of C. botulinum spores in soil and foods in the northern parts of China was 14.8 % , while it was only 2.5 % in the south .
	manualset3
115205	8	403479	5	NULL	NULL	0	NULL	2.5 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Nationwide surveys showed that the average detection rate of C. botulinum spores in soil and foods in the northern parts of China was 14.8 % , while it was only 2.5 % in the south .
	manualset3
115206	9	403479	5	NULL	NULL	0	NULL	south	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Nationwide surveys showed that the average detection rate of C. botulinum spores in soil and foods in the northern parts of China was 14.8 % , while it was only 2.5 % in the south .
	manualset3
115213	1	403480	5	NULL	NULL	0	NULL	Native heparin	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Native heparin and the derivatives were incubated with Flavobacterium heparinase II at 25 degrees C. The progress of degradation was followed by the delta A235 and the final composition examined by gel filtration with Bio-Gel P-4 .
	manualset3
115217	2	403480	5	NULL	NULL	0	NULL	derivatives	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Native heparin and the derivatives were incubated with Flavobacterium heparinase II at 25 degrees C. The progress of degradation was followed by the delta A235 and the final composition examined by gel filtration with Bio-Gel P-4 .
	manualset3
115220	3	403480	5	NULL	NULL	0	NULL	Flavobacterium heparinase II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Native heparin and the derivatives were incubated with Flavobacterium heparinase II at 25 degrees C. The progress of degradation was followed by the delta A235 and the final composition examined by gel filtration with Bio-Gel P-4 .
	manualset3
115221	4	403480	5	NULL	NULL	0	NULL	25 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Native heparin and the derivatives were incubated with Flavobacterium heparinase II at 25 degrees C. The progress of degradation was followed by the delta A235 and the final composition examined by gel filtration with Bio-Gel P-4 .
	manualset3
115222	5	403480	5	NULL	NULL	0	NULL	progress	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Native heparin and the derivatives were incubated with Flavobacterium heparinase II at 25 degrees C. The progress of degradation was followed by the delta A235 and the final composition examined by gel filtration with Bio-Gel P-4 .
	manualset3
115223	6	403480	5	NULL	NULL	0	NULL	degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Native heparin and the derivatives were incubated with Flavobacterium heparinase II at 25 degrees C. The progress of degradation was followed by the delta A235 and the final composition examined by gel filtration with Bio-Gel P-4 .
	manualset3
115224	7	403480	5	NULL	NULL	0	NULL	delta A235	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Native heparin and the derivatives were incubated with Flavobacterium heparinase II at 25 degrees C. The progress of degradation was followed by the delta A235 and the final composition examined by gel filtration with Bio-Gel P-4 .
	manualset3
115225	8	403480	5	NULL	NULL	0	NULL	final composition	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Native heparin and the derivatives were incubated with Flavobacterium heparinase II at 25 degrees C. The progress of degradation was followed by the delta A235 and the final composition examined by gel filtration with Bio-Gel P-4 .
	manualset3
115226	9	403480	5	NULL	NULL	0	NULL	gel filtration	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Native heparin and the derivatives were incubated with Flavobacterium heparinase II at 25 degrees C. The progress of degradation was followed by the delta A235 and the final composition examined by gel filtration with Bio-Gel P-4 .
	manualset3
115227	10	403480	5	NULL	NULL	0	NULL	Bio-Gel P-4	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Native heparin and the derivatives were incubated with Flavobacterium heparinase II at 25 degrees C. The progress of degradation was followed by the delta A235 and the final composition examined by gel filtration with Bio-Gel P-4 .
	manualset3
115244	1	403481	5	NULL	NULL	0	NULL	Natriuretic peptide ANP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Natriuretic peptides ANP , BNP and CNP with their receptors A , B , and C play an important role in maintaining the homeostasis .
	manualset3
115245	2	403481	5	NULL	NULL	NULL	NULL	Natriuretic peptide BNP	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Natriuretic peptides ANP , BNP and CNP with their receptors A , B , and C play an important role in maintaining the homeostasis .
	manualset3
115247	3	403481	5	NULL	NULL	0	NULL	Natriuretic peptide CNP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Natriuretic peptides ANP , BNP and CNP with their receptors A , B , and C play an important role in maintaining the homeostasis .
	manualset3
115251	4	403481	5	NULL	NULL	0	NULL	receptor A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Natriuretic peptides ANP , BNP and CNP with their receptors A , B , and C play an important role in maintaining the homeostasis .
	manualset3
115252	5	403481	5	NULL	NULL	0	NULL	receptor B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Natriuretic peptides ANP , BNP and CNP with their receptors A , B , and C play an important role in maintaining the homeostasis .
	manualset3
115253	6	403481	5	NULL	NULL	0	NULL	receptor C	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Natriuretic peptides ANP , BNP and CNP with their receptors A , B , and C play an important role in maintaining the homeostasis .
	manualset3
115255	7	403481	5	NULL	NULL	0	NULL	important role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Natriuretic peptides ANP , BNP and CNP with their receptors A , B , and C play an important role in maintaining the homeostasis .
	manualset3
115257	8	403481	5	NULL	NULL	0	NULL	homeostasis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Natriuretic peptides ANP , BNP and CNP with their receptors A , B , and C play an important role in maintaining the homeostasis .
	manualset3
115385	1	403482	5	NULL	NULL	0	NULL	Natural cycle in-vitro fertilization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural cycle in-vitro fertilization with embryo cryopreservation prior to chemotherapy for carcinoma of the breast .
	manualset3
115386	2	403482	5	NULL	NULL	0	NULL	embryo cryopreservation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural cycle in-vitro fertilization with embryo cryopreservation prior to chemotherapy for carcinoma of the breast .
	manualset3
115387	3	403482	5	NULL	NULL	0	NULL	chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural cycle in-vitro fertilization with embryo cryopreservation prior to chemotherapy for carcinoma of the breast .
	manualset3
115388	4	403482	5	NULL	NULL	NULL	NULL	carcinoma of the breast	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Natural cycle in-vitro fertilization with embryo cryopreservation prior to chemotherapy for carcinoma of the breast .
	manualset3
115390	1	403483	5	NULL	NULL	0	NULL	Natural eotaxin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural eotaxin is comprised of a mixture of N-terminal-truncated and O-glycosylated variants .
	manualset3
115391	2	403483	5	NULL	NULL	0	NULL	mixture	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural eotaxin is comprised of a mixture of N-terminal-truncated and O-glycosylated variants .
	manualset3
115392	3	403483	5	NULL	NULL	0	NULL	N-terminal-truncated variant	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural eotaxin is comprised of a mixture of N-terminal-truncated and O-glycosylated variants .
	manualset3
115393	4	403483	5	NULL	NULL	0	NULL	O-glycosylated variant	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural eotaxin is comprised of a mixture of N-terminal-truncated and O-glycosylated variants .
	manualset3
115394	1	403484	5	NULL	NULL	0	NULL	comparative study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative study of the submicroscopic reaction of hepatocytes of 3 groups of test dogs showed pronounced changes in the endoplasmatic reticulum : vacuolar transformation balloon dystrophy .
	manualset3
115395	2	403484	5	NULL	NULL	0	NULL	submicroscopic reaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative study of the submicroscopic reaction of hepatocytes of 3 groups of test dogs showed pronounced changes in the endoplasmatic reticulum : vacuolar transformation balloon dystrophy .
	manualset3
115396	3	403484	5	NULL	NULL	0	NULL	hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative study of the submicroscopic reaction of hepatocytes of 3 groups of test dogs showed pronounced changes in the endoplasmatic reticulum : vacuolar transformation balloon dystrophy .
	manualset3
115397	4	403484	5	NULL	NULL	0	NULL	 3 groups	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative study of the submicroscopic reaction of hepatocytes of 3 groups of test dogs showed pronounced changes in the endoplasmatic reticulum : vacuolar transformation balloon dystrophy .
	manualset3
115398	5	403484	5	NULL	NULL	0	NULL	test dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative study of the submicroscopic reaction of hepatocytes of 3 groups of test dogs showed pronounced changes in the endoplasmatic reticulum : vacuolar transformation balloon dystrophy .
	manualset3
115399	6	403484	5	NULL	NULL	0	NULL	changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative study of the submicroscopic reaction of hepatocytes of 3 groups of test dogs showed pronounced changes in the endoplasmatic reticulum : vacuolar transformation balloon dystrophy .
	manualset3
115400	7	403484	5	NULL	NULL	0	NULL	endoplasmatic reticulum	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative study of the submicroscopic reaction of hepatocytes of 3 groups of test dogs showed pronounced changes in the endoplasmatic reticulum : vacuolar transformation balloon dystrophy .
	manualset3
115401	8	403484	5	NULL	NULL	0	NULL	vacuolar transformation balloon dystrophy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative study of the submicroscopic reaction of hepatocytes of 3 groups of test dogs showed pronounced changes in the endoplasmatic reticulum : vacuolar transformation balloon dystrophy .
	manualset3
115402	1	403485	5	NULL	NULL	0	NULL	Natural history	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural history of left ventricular mechanics in transplanted hearts : relationships with clinical variables and genetic expression profiles of allograft rejection .
	manualset3
115403	2	403485	5	NULL	NULL	0	NULL	left ventricular mechanics	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural history of left ventricular mechanics in transplanted hearts : relationships with clinical variables and genetic expression profiles of allograft rejection .
	manualset3
115404	3	403485	5	NULL	NULL	0	NULL	transplanted hearts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural history of left ventricular mechanics in transplanted hearts : relationships with clinical variables and genetic expression profiles of allograft rejection .
	manualset3
115405	4	403485	5	NULL	NULL	0	NULL	relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural history of left ventricular mechanics in transplanted hearts : relationships with clinical variables and genetic expression profiles of allograft rejection .
	manualset3
115406	5	403485	5	NULL	NULL	0	NULL	clinical variables 	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural history of left ventricular mechanics in transplanted hearts : relationships with clinical variables and genetic expression profiles of allograft rejection .
	manualset3
115407	6	403485	5	NULL	NULL	0	NULL	genetic expression profiles	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural history of left ventricular mechanics in transplanted hearts : relationships with clinical variables and genetic expression profiles of allograft rejection .
	manualset3
115408	7	403485	5	NULL	NULL	0	NULL	allograft rejection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural history of left ventricular mechanics in transplanted hearts : relationships with clinical variables and genetic expression profiles of allograft rejection .
	manualset3
115409	1	403486	5	NULL	NULL	0	NULL	Natural infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural infection with zoonotic subtype of Cryptosporidium parvum in Capybara ( Hydrochoerus hydrochaeris ) from Brazil .
	manualset3
115410	2	403486	5	NULL	NULL	0	NULL	zoonotic subtype of Cryptosporidium parvum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural infection with zoonotic subtype of Cryptosporidium parvum in Capybara ( Hydrochoerus hydrochaeris ) from Brazil .
	manualset3
115411	3	403486	5	NULL	NULL	0	NULL	Capybara ( Hydrochoerus hydrochaeris )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural infection with zoonotic subtype of Cryptosporidium parvum in Capybara ( Hydrochoerus hydrochaeris ) from Brazil .
	manualset3
115412	4	403486	5	NULL	NULL	0	NULL	Brazil	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural infection with zoonotic subtype of Cryptosporidium parvum in Capybara ( Hydrochoerus hydrochaeris ) from Brazil .
	manualset3
115413	1	403487	5	NULL	NULL	0	NULL	Natural killer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural killer cells ameliorate liver fibrosis by killing activated stellate cells in NKG2D-dependent and tumor necrosis factor-related apoptosis-inducing ligand-dependent manners .
	manualset3
115414	2	403487	5	NULL	NULL	0	NULL	liver fibrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural killer cells ameliorate liver fibrosis by killing activated stellate cells in NKG2D-dependent and tumor necrosis factor-related apoptosis-inducing ligand-dependent manners .
	manualset3
115415	3	403487	5	NULL	NULL	0	NULL	activated stellate cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural killer cells ameliorate liver fibrosis by killing activated stellate cells in NKG2D-dependent and tumor necrosis factor-related apoptosis-inducing ligand-dependent manners .
	manualset3
115416	4	403487	5	NULL	NULL	NULL	NULL	NKG2D-dependent manners	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Natural killer cells ameliorate liver fibrosis by killing activated stellate cells in NKG2D-dependent and tumor necrosis factor-related apoptosis-inducing ligand-dependent manners .
	manualset3
115418	5	403487	5	NULL	NULL	0	NULL	tumor necrosis factor-related apoptosis-inducing ligand-dependent manners	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural killer cells ameliorate liver fibrosis by killing activated stellate cells in NKG2D-dependent and tumor necrosis factor-related apoptosis-inducing ligand-dependent manners .
	manualset3
115419	1	403488	5	NULL	NULL	0	NULL	Natural killer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural killer cells are important players of the innate immunity .
	manualset3
115420	2	403488	5	NULL	NULL	0	NULL	important players	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural killer cells are important players of the innate immunity .
	manualset3
115421	3	403488	5	NULL	NULL	0	NULL	innate immunity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural killer cells are important players of the innate immunity .
	manualset3
115422	1	403489	5	NULL	NULL	0	NULL	antimutagenic compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Naturally occurring antimutagenic compounds are extensively analyzed for their capacity to protect cells from induced damage .
	manualset3
115423	2	403489	5	NULL	NULL	0	NULL	capacity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Naturally occurring antimutagenic compounds are extensively analyzed for their capacity to protect cells from induced damage .
	manualset3
115424	3	403489	5	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Naturally occurring antimutagenic compounds are extensively analyzed for their capacity to protect cells from induced damage .
	manualset3
115425	4	403489	5	NULL	NULL	0	NULL	induced damage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Naturally occurring antimutagenic compounds are extensively analyzed for their capacity to protect cells from induced damage .
	manualset3
115426	1	403490	5	NULL	NULL	0	NULL	Ndufs6 ( gt/gt ) mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ndufs6 ( gt/gt ) mice are born healthy , attain normal weight and maturity , and are fertile .
	manualset3
115427	2	403490	5	NULL	NULL	0	NULL	healthy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ndufs6 ( gt/gt ) mice are born healthy , attain normal weight and maturity , and are fertile .
	manualset3
115428	3	403490	5	NULL	NULL	0	NULL	normal weight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ndufs6 ( gt/gt ) mice are born healthy , attain normal weight and maturity , and are fertile .
	manualset3
115429	4	403490	5	NULL	NULL	0	NULL	maturity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ndufs6 ( gt/gt ) mice are born healthy , attain normal weight and maturity , and are fertile .
	manualset3
115431	1	403491	5	NULL	NULL	0	NULL	comparative study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative study of the susceptibility to major and minor drugs of tubercle bacilli isolated from 100 consecutive patients never treated with minor drugs .
	manualset3
115432	2	403491	5	NULL	NULL	0	NULL	susceptibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative study of the susceptibility to major and minor drugs of tubercle bacilli isolated from 100 consecutive patients never treated with minor drugs .
	manualset3
115433	3	403491	5	NULL	NULL	0	NULL	major and minor drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative study of the susceptibility to major and minor drugs of tubercle bacilli isolated from 100 consecutive patients never treated with minor drugs .
	manualset3
115434	4	403491	5	NULL	NULL	0	NULL	tubercle bacilli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative study of the susceptibility to major and minor drugs of tubercle bacilli isolated from 100 consecutive patients never treated with minor drugs .
	manualset3
115435	5	403491	5	NULL	NULL	0	NULL	100 consecutive patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative study of the susceptibility to major and minor drugs of tubercle bacilli isolated from 100 consecutive patients never treated with minor drugs .
	manualset3
115436	6	403491	5	NULL	NULL	0	NULL	minor drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative study of the susceptibility to major and minor drugs of tubercle bacilli isolated from 100 consecutive patients never treated with minor drugs .
	manualset3
115437	1	403492	5	NULL	NULL	0	NULL	smelter	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Near the smelter , the Pb concentration of the endogeic Aporrectodea caliginosa was higher than in the epigeic Lumbricus rubellus and L. casteneus .
	manualset3
115438	2	403492	5	NULL	NULL	0	NULL	Pb concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Near the smelter , the Pb concentration of the endogeic Aporrectodea caliginosa was higher than in the epigeic Lumbricus rubellus and L. casteneus .
	manualset3
115439	3	403492	5	NULL	NULL	0	NULL	endogeic Aporrectodea caliginosa	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Near the smelter , the Pb concentration of the endogeic Aporrectodea caliginosa was higher than in the epigeic Lumbricus rubellus and L. casteneus .
	manualset3
115440	4	403492	5	NULL	NULL	0	NULL	epigeic Lumbricus rubellus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Near the smelter , the Pb concentration of the endogeic Aporrectodea caliginosa was higher than in the epigeic Lumbricus rubellus and L. casteneus .
	manualset3
115441	5	403492	5	NULL	NULL	0	NULL	L. casteneus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Near the smelter , the Pb concentration of the endogeic Aporrectodea caliginosa was higher than in the epigeic Lumbricus rubellus and L. casteneus .
	manualset3
115442	1	403493	5	NULL	NULL	0	NULL	150 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Nearly 150 leading FRDA scientists from around the world discussed their new insights and findings .
	manualset3
115443	2	403493	5	NULL	NULL	0	NULL	FRDA scientists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nearly 150 leading FRDA scientists from around the world discussed their new insights and findings .
	manualset3
115444	3	403493	5	NULL	NULL	0	NULL	world	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Nearly 150 leading FRDA scientists from around the world discussed their new insights and findings .
	manualset3
115445	4	403493	5	NULL	NULL	0	NULL	new insights	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nearly 150 leading FRDA scientists from around the world discussed their new insights and findings .
	manualset3
115446	5	403493	5	NULL	NULL	0	NULL	findings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nearly 150 leading FRDA scientists from around the world discussed their new insights and findings .
	manualset3
115474	1	403494	5	NULL	NULL	0	NULL	tolerance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nearly complete tolerance to a test dose of 50 micrograms/kg of LSD occurred within 24 h following an initial dose of 50 micrograms/kg of the drug , using limb flicking and abortive grooming as as behavioral indices in the cat .
	manualset3
115475	2	403494	5	NULL	NULL	0	NULL	test dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nearly complete tolerance to a test dose of 50 micrograms/kg of LSD occurred within 24 h following an initial dose of 50 micrograms/kg of the drug , using limb flicking and abortive grooming as as behavioral indices in the cat .
	manualset3
115476	3	403494	5	NULL	NULL	0	NULL	50 micrograms/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Nearly complete tolerance to a test dose of 50 micrograms/kg of LSD occurred within 24 h following an initial dose of 50 micrograms/kg of the drug , using limb flicking and abortive grooming as as behavioral indices in the cat .
	manualset3
115477	4	403494	5	NULL	NULL	0	NULL	LSD	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Nearly complete tolerance to a test dose of 50 micrograms/kg of LSD occurred within 24 h following an initial dose of 50 micrograms/kg of the drug , using limb flicking and abortive grooming as as behavioral indices in the cat .
	manualset3
115478	5	403494	5	NULL	NULL	0	NULL	24 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Nearly complete tolerance to a test dose of 50 micrograms/kg of LSD occurred within 24 h following an initial dose of 50 micrograms/kg of the drug , using limb flicking and abortive grooming as as behavioral indices in the cat .
	manualset3
115479	6	403494	5	NULL	NULL	0	NULL	initial dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nearly complete tolerance to a test dose of 50 micrograms/kg of LSD occurred within 24 h following an initial dose of 50 micrograms/kg of the drug , using limb flicking and abortive grooming as as behavioral indices in the cat .
	manualset3
115480	7	403494	5	NULL	NULL	0	NULL	50 micrograms/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Nearly complete tolerance to a test dose of 50 micrograms/kg of LSD occurred within 24 h following an initial dose of 50 micrograms/kg of the drug , using limb flicking and abortive grooming as as behavioral indices in the cat .
	manualset3
115481	8	403494	5	NULL	NULL	0	NULL	drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Nearly complete tolerance to a test dose of 50 micrograms/kg of LSD occurred within 24 h following an initial dose of 50 micrograms/kg of the drug , using limb flicking and abortive grooming as as behavioral indices in the cat .
	manualset3
115482	9	403494	5	NULL	NULL	0	NULL	limb flicking	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nearly complete tolerance to a test dose of 50 micrograms/kg of LSD occurred within 24 h following an initial dose of 50 micrograms/kg of the drug , using limb flicking and abortive grooming as as behavioral indices in the cat .
	manualset3
115483	10	403494	5	NULL	NULL	0	NULL	abortive grooming	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nearly complete tolerance to a test dose of 50 micrograms/kg of LSD occurred within 24 h following an initial dose of 50 micrograms/kg of the drug , using limb flicking and abortive grooming as as behavioral indices in the cat .
	manualset3
115484	11	403494	5	NULL	NULL	0	NULL	behavioral indices	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nearly complete tolerance to a test dose of 50 micrograms/kg of LSD occurred within 24 h following an initial dose of 50 micrograms/kg of the drug , using limb flicking and abortive grooming as as behavioral indices in the cat .
	manualset3
115485	12	403494	5	NULL	NULL	0	NULL	cat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Nearly complete tolerance to a test dose of 50 micrograms/kg of LSD occurred within 24 h following an initial dose of 50 micrograms/kg of the drug , using limb flicking and abortive grooming as as behavioral indices in the cat .
	manualset3
115486	1	403495	5	NULL	NULL	0	NULL	identical results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Nearly identical results were obtained for the elementary quaternary ligand tetramethylammonium , indicating that these tyrosines contribute to stabilization of the quaternary ammonium portion of agonist .
	manualset3
115487	2	403495	5	NULL	NULL	0	NULL	elementary quaternary ligand tetramethylammonium	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Nearly identical results were obtained for the elementary quaternary ligand tetramethylammonium , indicating that these tyrosines contribute to stabilization of the quaternary ammonium portion of agonist .
	manualset3
115488	3	403495	5	NULL	NULL	0	NULL	tyrosines	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Nearly identical results were obtained for the elementary quaternary ligand tetramethylammonium , indicating that these tyrosines contribute to stabilization of the quaternary ammonium portion of agonist .
	manualset3
115489	4	403495	5	NULL	NULL	0	NULL	stabilization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nearly identical results were obtained for the elementary quaternary ligand tetramethylammonium , indicating that these tyrosines contribute to stabilization of the quaternary ammonium portion of agonist .
	manualset3
115490	5	403495	5	NULL	NULL	0	NULL	quaternary ammonium portion	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Nearly identical results were obtained for the elementary quaternary ligand tetramethylammonium , indicating that these tyrosines contribute to stabilization of the quaternary ammonium portion of agonist .
	manualset3
115491	6	403495	5	NULL	NULL	0	NULL	agonist	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nearly identical results were obtained for the elementary quaternary ligand tetramethylammonium , indicating that these tyrosines contribute to stabilization of the quaternary ammonium portion of agonist .
	manualset3
115492	1	403496	5	NULL	NULL	0	NULL	Necrosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Necrosis of the grafts was seen after the 7th POD in Group B. CD8 positive cells were observed in the perivascular region of the grafts of Group B and they were increasing after the 2nd POD .
	manualset3
115493	2	403496	5	NULL	NULL	NULL	NULL	grafts	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Necrosis of the grafts was seen after the 7th POD in Group B. CD8 positive cells were observed in the perivascular region of the grafts of Group B and they were increasing after the 2nd POD .
	manualset3
115494	3	403496	5	NULL	NULL	0	NULL	7th POD 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Necrosis of the grafts was seen after the 7th POD in Group B. CD8 positive cells were observed in the perivascular region of the grafts of Group B and they were increasing after the 2nd POD .
	manualset3
115495	4	403496	5	NULL	NULL	0	NULL	Group B	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Necrosis of the grafts was seen after the 7th POD in Group B. CD8 positive cells were observed in the perivascular region of the grafts of Group B and they were increasing after the 2nd POD .
	manualset3
115496	5	403496	5	NULL	NULL	0	NULL	CD8 positive cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Necrosis of the grafts was seen after the 7th POD in Group B. CD8 positive cells were observed in the perivascular region of the grafts of Group B and they were increasing after the 2nd POD .
	manualset3
115497	6	403496	5	NULL	NULL	0	NULL	perivascular region	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Necrosis of the grafts was seen after the 7th POD in Group B. CD8 positive cells were observed in the perivascular region of the grafts of Group B and they were increasing after the 2nd POD .
	manualset3
115498	7	403496	5	NULL	NULL	0	NULL	grafts	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Necrosis of the grafts was seen after the 7th POD in Group B. CD8 positive cells were observed in the perivascular region of the grafts of Group B and they were increasing after the 2nd POD .
	manualset3
115499	8	403496	5	NULL	NULL	0	NULL	Group B	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Necrosis of the grafts was seen after the 7th POD in Group B. CD8 positive cells were observed in the perivascular region of the grafts of Group B and they were increasing after the 2nd POD .
	manualset3
115500	9	403496	5	NULL	NULL	0	NULL	2nd POD	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Necrosis of the grafts was seen after the 7th POD in Group B. CD8 positive cells were observed in the perivascular region of the grafts of Group B and they were increasing after the 2nd POD .
	manualset3
115501	1	403497	5	NULL	NULL	0	NULL	Necrotizing myopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Necrotizing myopathy induced by overexpression of interferon-gamma in transgenic mice .
	manualset3
115502	2	403497	5	NULL	NULL	0	NULL	overexpression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Necrotizing myopathy induced by overexpression of interferon-gamma in transgenic mice .
	manualset3
115503	3	403497	5	NULL	NULL	0	NULL	interferon-gamma	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Necrotizing myopathy induced by overexpression of interferon-gamma in transgenic mice .
	manualset3
115504	4	403497	5	NULL	NULL	0	NULL	transgenic mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Necrotizing myopathy induced by overexpression of interferon-gamma in transgenic mice .
	manualset3
115505	1	403498	5	NULL	NULL	NULL	NULL	assessment	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Needs assessment : a tool for hospice expansion .
	manualset3
115506	2	403498	5	NULL	NULL	0	NULL	tool	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Needs assessment : a tool for hospice expansion .
	manualset3
115507	3	403498	5	NULL	NULL	0	NULL	hospice expansion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Needs assessment : a tool for hospice expansion .
	manualset3
115508	1	403499	5	NULL	NULL	0	NULL	aftereffects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Negative aftereffects observed in imagined motion imply that the imagination represents movement as an inference from position changes of static images .
	manualset3
115509	2	403499	5	NULL	NULL	0	NULL	imagined motion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Negative aftereffects observed in imagined motion imply that the imagination represents movement as an inference from position changes of static images .
	manualset3
115510	3	403499	5	NULL	NULL	0	NULL	imagination	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Negative aftereffects observed in imagined motion imply that the imagination represents movement as an inference from position changes of static images .
	manualset3
115511	4	403499	5	NULL	NULL	0	NULL	movement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Negative aftereffects observed in imagined motion imply that the imagination represents movement as an inference from position changes of static images .
	manualset3
115514	5	403499	5	NULL	NULL	0	NULL	inference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Negative aftereffects observed in imagined motion imply that the imagination represents movement as an inference from position changes of static images .
	manualset3
115517	6	403499	5	NULL	NULL	0	NULL	position changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Negative aftereffects observed in imagined motion imply that the imagination represents movement as an inference from position changes of static images .
	manualset3
115521	7	403499	5	NULL	NULL	0	NULL	static images	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Negative aftereffects observed in imagined motion imply that the imagination represents movement as an inference from position changes of static images .
	manualset3
115523	1	403500	5	NULL	NULL	0	NULL	Biochemical research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Biochemical research on hibernation ) .
	manualset3
115524	2	403500	5	NULL	NULL	0	NULL	hibernation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Biochemical research on hibernation ) .
	manualset3
115525	1	403501	5	NULL	NULL	0	NULL	part	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neglecting this part of the duty to provide appropriate care brings moral anguish to all participants in the peculiar circumstances that have come to surround death in the ICUs of developed countries .
	manualset3
115526	2	403501	5	NULL	NULL	0	NULL	duty	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neglecting this part of the duty to provide appropriate care brings moral anguish to all participants in the peculiar circumstances that have come to surround death in the ICUs of developed countries .
	manualset3
115527	3	403501	5	NULL	NULL	0	NULL	care	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neglecting this part of the duty to provide appropriate care brings moral anguish to all participants in the peculiar circumstances that have come to surround death in the ICUs of developed countries .
	manualset3
115531	4	403501	5	NULL	NULL	0	NULL	moral anguish	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neglecting this part of the duty to provide appropriate care brings moral anguish to all participants in the peculiar circumstances that have come to surround death in the ICUs of developed countries .
	manualset3
115533	5	403501	5	NULL	NULL	0	NULL	participants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Neglecting this part of the duty to provide appropriate care brings moral anguish to all participants in the peculiar circumstances that have come to surround death in the ICUs of developed countries .
	manualset3
115534	6	403501	5	NULL	NULL	0	NULL	peculiar circumstances	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neglecting this part of the duty to provide appropriate care brings moral anguish to all participants in the peculiar circumstances that have come to surround death in the ICUs of developed countries .
	manualset3
115535	7	403501	5	NULL	NULL	0	NULL	death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neglecting this part of the duty to provide appropriate care brings moral anguish to all participants in the peculiar circumstances that have come to surround death in the ICUs of developed countries .
	manualset3
115536	8	403501	5	NULL	NULL	0	NULL	ICUs	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Neglecting this part of the duty to provide appropriate care brings moral anguish to all participants in the peculiar circumstances that have come to surround death in the ICUs of developed countries .
	manualset3
115538	9	403501	5	NULL	NULL	0	NULL	developed countries	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Neglecting this part of the duty to provide appropriate care brings moral anguish to all participants in the peculiar circumstances that have come to surround death in the ICUs of developed countries .
	manualset3
115543	1	403502	5	NULL	NULL	NULL	NULL	anti-IL-12 neutralizing antibody	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Neither the anti-IL-12 neutralizing antibody nor the delivery of exogenous IL-12 from microspheres had any effect on tumor xenografts in the absence of the inflammatory leukocytes .
	manualset3
115544	2	403502	5	NULL	NULL	0	NULL	delivery	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the anti-IL-12 neutralizing antibody nor the delivery of exogenous IL-12 from microspheres had any effect on tumor xenografts in the absence of the inflammatory leukocytes .
	manualset3
115545	3	403502	5	NULL	NULL	0	NULL	exogenous IL-12	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the anti-IL-12 neutralizing antibody nor the delivery of exogenous IL-12 from microspheres had any effect on tumor xenografts in the absence of the inflammatory leukocytes .
	manualset3
115547	4	403502	5	NULL	NULL	0	NULL	microspheres	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the anti-IL-12 neutralizing antibody nor the delivery of exogenous IL-12 from microspheres had any effect on tumor xenografts in the absence of the inflammatory leukocytes .
	manualset3
115549	5	403502	5	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the anti-IL-12 neutralizing antibody nor the delivery of exogenous IL-12 from microspheres had any effect on tumor xenografts in the absence of the inflammatory leukocytes .
	manualset3
115551	6	403502	5	NULL	NULL	0	NULL	tumor xenografts	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the anti-IL-12 neutralizing antibody nor the delivery of exogenous IL-12 from microspheres had any effect on tumor xenografts in the absence of the inflammatory leukocytes .
	manualset3
115552	7	403502	5	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the anti-IL-12 neutralizing antibody nor the delivery of exogenous IL-12 from microspheres had any effect on tumor xenografts in the absence of the inflammatory leukocytes .
	manualset3
115553	8	403502	5	NULL	NULL	0	NULL	inflammatory leukocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the anti-IL-12 neutralizing antibody nor the delivery of exogenous IL-12 from microspheres had any effect on tumor xenografts in the absence of the inflammatory leukocytes .
	manualset3
115572	1	403503	5	NULL	NULL	0	NULL	malnutrition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the malnutrition nor the liver damage of the mothers are necessary presuppositions .
	manualset3
115573	2	403503	5	NULL	NULL	0	NULL	liver damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the malnutrition nor the liver damage of the mothers are necessary presuppositions .
	manualset3
115574	3	403503	5	NULL	NULL	0	NULL	mothers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the malnutrition nor the liver damage of the mothers are necessary presuppositions .
	manualset3
115577	4	403503	5	NULL	NULL	0	NULL	presuppositions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the malnutrition nor the liver damage of the mothers are necessary presuppositions .
	manualset3
115580	1	403504	5	NULL	NULL	0	NULL	organization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the organization of the adult nor the modalities of development are encoded in the DNA .
	manualset3
115583	2	403504	5	NULL	NULL	NULL	NULL	adult	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Neither the organization of the adult nor the modalities of development are encoded in the DNA .
	manualset3
115588	3	403504	5	NULL	NULL	0	NULL	modalities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the organization of the adult nor the modalities of development are encoded in the DNA .
	manualset3
115590	4	403504	5	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the organization of the adult nor the modalities of development are encoded in the DNA .
	manualset3
115591	5	403504	5	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the organization of the adult nor the modalities of development are encoded in the DNA .
	manualset3
115594	1	403505	5	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the presence of circulating heartworm antibodies and antigen nor the presence of antigenuria predicted the development of proteinuria .
	manualset3
115597	2	403505	5	NULL	NULL	0	NULL	circulating heartworm antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the presence of circulating heartworm antibodies and antigen nor the presence of antigenuria predicted the development of proteinuria .
	manualset3
115599	3	403505	5	NULL	NULL	0	NULL	antigen	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the presence of circulating heartworm antibodies and antigen nor the presence of antigenuria predicted the development of proteinuria .
	manualset3
115600	4	403505	5	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the presence of circulating heartworm antibodies and antigen nor the presence of antigenuria predicted the development of proteinuria .
	manualset3
115604	5	403505	5	NULL	NULL	0	NULL	antigenuria	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the presence of circulating heartworm antibodies and antigen nor the presence of antigenuria predicted the development of proteinuria .
	manualset3
115608	6	403505	5	NULL	NULL	0	NULL	development	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the presence of circulating heartworm antibodies and antigen nor the presence of antigenuria predicted the development of proteinuria .
	manualset3
115611	7	403505	5	NULL	NULL	0	NULL	proteinuria	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the presence of circulating heartworm antibodies and antigen nor the presence of antigenuria predicted the development of proteinuria .
	manualset3
115613	1	403506	5	NULL	NULL	0	NULL	secondary structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the secondary structure , nor the oxidation-reduction midpoint potential ( Em ) values of the siroheme and ( 4Fe-4S ) cluster prosthetic groups of sulfite reductase , nor the binding affinity of the enzyme for ferredoxin were affected by NBS treatment .
	manualset3
115615	2	403506	5	NULL	NULL	0	NULL	oxidation-reduction midpoint potential ( Em ) values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the secondary structure , nor the oxidation-reduction midpoint potential ( Em ) values of the siroheme and ( 4Fe-4S ) cluster prosthetic groups of sulfite reductase , nor the binding affinity of the enzyme for ferredoxin were affected by NBS treatment .
	manualset3
115631	3	403506	5	NULL	NULL	0	NULL	siroheme	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the secondary structure , nor the oxidation-reduction midpoint potential ( Em ) values of the siroheme and ( 4Fe-4S ) cluster prosthetic groups of sulfite reductase , nor the binding affinity of the enzyme for ferredoxin were affected by NBS treatment .
	manualset3
115632	4	403506	5	NULL	NULL	0	NULL	( 4Fe-4S ) cluster prosthetic groups 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the secondary structure , nor the oxidation-reduction midpoint potential ( Em ) values of the siroheme and ( 4Fe-4S ) cluster prosthetic groups of sulfite reductase , nor the binding affinity of the enzyme for ferredoxin were affected by NBS treatment .
	manualset3
115633	5	403506	5	NULL	NULL	0	NULL	sulfite reductase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the secondary structure , nor the oxidation-reduction midpoint potential ( Em ) values of the siroheme and ( 4Fe-4S ) cluster prosthetic groups of sulfite reductase , nor the binding affinity of the enzyme for ferredoxin were affected by NBS treatment .
	manualset3
115638	6	403506	5	NULL	NULL	0	NULL	binding affinity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the secondary structure , nor the oxidation-reduction midpoint potential ( Em ) values of the siroheme and ( 4Fe-4S ) cluster prosthetic groups of sulfite reductase , nor the binding affinity of the enzyme for ferredoxin were affected by NBS treatment .
	manualset3
115640	7	403506	5	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the secondary structure , nor the oxidation-reduction midpoint potential ( Em ) values of the siroheme and ( 4Fe-4S ) cluster prosthetic groups of sulfite reductase , nor the binding affinity of the enzyme for ferredoxin were affected by NBS treatment .
	manualset3
115642	8	403506	5	NULL	NULL	0	NULL	ferredoxin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the secondary structure , nor the oxidation-reduction midpoint potential ( Em ) values of the siroheme and ( 4Fe-4S ) cluster prosthetic groups of sulfite reductase , nor the binding affinity of the enzyme for ferredoxin were affected by NBS treatment .
	manualset3
115643	9	403506	5	NULL	NULL	0	NULL	NBS treatment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the secondary structure , nor the oxidation-reduction midpoint potential ( Em ) values of the siroheme and ( 4Fe-4S ) cluster prosthetic groups of sulfite reductase , nor the binding affinity of the enzyme for ferredoxin were affected by NBS treatment .
	manualset3
115774	1	403507	5	NULL	NULL	0	NULL	serum levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither were they related to the serum levels of copper , globulins , or predisposition to hepatic encephalopathy .
	manualset3
115775	2	403507	5	NULL	NULL	0	NULL	copper	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither were they related to the serum levels of copper , globulins , or predisposition to hepatic encephalopathy .
	manualset3
115776	3	403507	5	NULL	NULL	0	NULL	globulins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither were they related to the serum levels of copper , globulins , or predisposition to hepatic encephalopathy .
	manualset3
115777	4	403507	5	NULL	NULL	NULL	NULL	predisposition	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Neither were they related to the serum levels of copper , globulins , or predisposition to hepatic encephalopathy .
	manualset3
115778	5	403507	5	NULL	NULL	0	NULL	hepatic encephalopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither were they related to the serum levels of copper , globulins , or predisposition to hepatic encephalopathy .
	manualset3
115779	1	403508	5	NULL	NULL	0	NULL	Rec12 ( Spo11 ortholog )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither Rec12 ( Spo11 ortholog ) nor I-SceI-induced breakage at mbs1 was significantly associated with crossing over in an apparently break-free interval ) 25 kb away .
	manualset3
115780	2	403508	5	NULL	NULL	0	NULL	I-SceI-induced breakage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither Rec12 ( Spo11 ortholog ) nor I-SceI-induced breakage at mbs1 was significantly associated with crossing over in an apparently break-free interval ) 25 kb away .
	manualset3
115781	3	403508	5	NULL	NULL	0	NULL	mbs1	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither Rec12 ( Spo11 ortholog ) nor I-SceI-induced breakage at mbs1 was significantly associated with crossing over in an apparently break-free interval ) 25 kb away .
	manualset3
115782	4	403508	5	NULL	NULL	0	NULL	crossing over	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither Rec12 ( Spo11 ortholog ) nor I-SceI-induced breakage at mbs1 was significantly associated with crossing over in an apparently break-free interval ) 25 kb away .
	manualset3
115783	5	403508	5	NULL	NULL	0	NULL	break-free interval	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither Rec12 ( Spo11 ortholog ) nor I-SceI-induced breakage at mbs1 was significantly associated with crossing over in an apparently break-free interval ) 25 kb away .
	manualset3
115784	6	403508	5	NULL	NULL	0	NULL	25 kb	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither Rec12 ( Spo11 ortholog ) nor I-SceI-induced breakage at mbs1 was significantly associated with crossing over in an apparently break-free interval ) 25 kb away .
	manualset3
115785	1	403509	5	NULL	NULL	0	NULL	naloxone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither naloxone ( 6 mg/h ) nor naloxonazine ( 34 mg ) had any effect on the total number of diaphragmatic electromyogram bursts per hour , mean instantaneous breathing rate , or incidence of breathing .
	manualset3
115786	2	403509	5	NULL	NULL	0	NULL	6 mg/h	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither naloxone ( 6 mg/h ) nor naloxonazine ( 34 mg ) had any effect on the total number of diaphragmatic electromyogram bursts per hour , mean instantaneous breathing rate , or incidence of breathing .
	manualset3
115787	3	403509	5	NULL	NULL	0	NULL	naloxonazine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither naloxone ( 6 mg/h ) nor naloxonazine ( 34 mg ) had any effect on the total number of diaphragmatic electromyogram bursts per hour , mean instantaneous breathing rate , or incidence of breathing .
	manualset3
115788	4	403509	5	NULL	NULL	0	NULL	34 mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither naloxone ( 6 mg/h ) nor naloxonazine ( 34 mg ) had any effect on the total number of diaphragmatic electromyogram bursts per hour , mean instantaneous breathing rate , or incidence of breathing .
	manualset3
115789	5	403509	5	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither naloxone ( 6 mg/h ) nor naloxonazine ( 34 mg ) had any effect on the total number of diaphragmatic electromyogram bursts per hour , mean instantaneous breathing rate , or incidence of breathing .
	manualset3
115790	6	403509	5	NULL	NULL	0	NULL	total number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither naloxone ( 6 mg/h ) nor naloxonazine ( 34 mg ) had any effect on the total number of diaphragmatic electromyogram bursts per hour , mean instantaneous breathing rate , or incidence of breathing .
	manualset3
115791	7	403509	5	NULL	NULL	0	NULL	diaphragmatic electromyogram bursts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither naloxone ( 6 mg/h ) nor naloxonazine ( 34 mg ) had any effect on the total number of diaphragmatic electromyogram bursts per hour , mean instantaneous breathing rate , or incidence of breathing .
	manualset3
115792	8	403509	5	NULL	NULL	0	NULL	hour	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither naloxone ( 6 mg/h ) nor naloxonazine ( 34 mg ) had any effect on the total number of diaphragmatic electromyogram bursts per hour , mean instantaneous breathing rate , or incidence of breathing .
	manualset3
115793	9	403509	5	NULL	NULL	0	NULL	breathing rate 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither naloxone ( 6 mg/h ) nor naloxonazine ( 34 mg ) had any effect on the total number of diaphragmatic electromyogram bursts per hour , mean instantaneous breathing rate , or incidence of breathing .
	manualset3
115794	10	403509	5	NULL	NULL	0	NULL	incidence	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither naloxone ( 6 mg/h ) nor naloxonazine ( 34 mg ) had any effect on the total number of diaphragmatic electromyogram bursts per hour , mean instantaneous breathing rate , or incidence of breathing .
	manualset3
115795	11	403509	5	NULL	NULL	0	NULL	breathing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither naloxone ( 6 mg/h ) nor naloxonazine ( 34 mg ) had any effect on the total number of diaphragmatic electromyogram bursts per hour , mean instantaneous breathing rate , or incidence of breathing .
	manualset3
115796	1	403510	5	NULL	NULL	0	NULL	EGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither EGF nor TGF-alpha increased transcription rates of IL-1 alpha , IL-1 beta , and IL-6 genes , but rather both EGF and TGF-alpha increased cytokine mRNA stability .
	manualset3
115797	2	403510	5	NULL	NULL	0	NULL	TGF-alpha 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither EGF nor TGF-alpha increased transcription rates of IL-1 alpha , IL-1 beta , and IL-6 genes , but rather both EGF and TGF-alpha increased cytokine mRNA stability .
	manualset3
115798	3	403510	5	NULL	NULL	0	NULL	transcription rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither EGF nor TGF-alpha increased transcription rates of IL-1 alpha , IL-1 beta , and IL-6 genes , but rather both EGF and TGF-alpha increased cytokine mRNA stability .
	manualset3
115799	4	403510	5	NULL	NULL	0	NULL	IL-1 alpha gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither EGF nor TGF-alpha increased transcription rates of IL-1 alpha , IL-1 beta , and IL-6 genes , but rather both EGF and TGF-alpha increased cytokine mRNA stability .
	manualset3
115800	5	403510	5	NULL	NULL	0	NULL	IL-1 beta gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither EGF nor TGF-alpha increased transcription rates of IL-1 alpha , IL-1 beta , and IL-6 genes , but rather both EGF and TGF-alpha increased cytokine mRNA stability .
	manualset3
115801	6	403510	5	NULL	NULL	0	NULL	IL-6 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither EGF nor TGF-alpha increased transcription rates of IL-1 alpha , IL-1 beta , and IL-6 genes , but rather both EGF and TGF-alpha increased cytokine mRNA stability .
	manualset3
115802	7	403510	5	NULL	NULL	0	NULL	EGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither EGF nor TGF-alpha increased transcription rates of IL-1 alpha , IL-1 beta , and IL-6 genes , but rather both EGF and TGF-alpha increased cytokine mRNA stability .
	manualset3
115803	8	403510	5	NULL	NULL	0	NULL	TGF-alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither EGF nor TGF-alpha increased transcription rates of IL-1 alpha , IL-1 beta , and IL-6 genes , but rather both EGF and TGF-alpha increased cytokine mRNA stability .
	manualset3
115804	9	403510	5	NULL	NULL	0	NULL	cytokine mRNA stability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither EGF nor TGF-alpha increased transcription rates of IL-1 alpha , IL-1 beta , and IL-6 genes , but rather both EGF and TGF-alpha increased cytokine mRNA stability .
	manualset3
115805	1	403511	5	NULL	NULL	0	NULL	comparison	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison across cycles confirmed the hypothesis that higher ovarian steroid levels are associated with an increased probability of conception .
	manualset3
115806	2	403511	5	NULL	NULL	NULL	NULL	cycles	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A comparison across cycles confirmed the hypothesis that higher ovarian steroid levels are associated with an increased probability of conception .
	manualset3
115807	3	403511	5	NULL	NULL	0	NULL	hypothesis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison across cycles confirmed the hypothesis that higher ovarian steroid levels are associated with an increased probability of conception .
	manualset3
115808	4	403511	5	NULL	NULL	0	NULL	higher ovarian steroid levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison across cycles confirmed the hypothesis that higher ovarian steroid levels are associated with an increased probability of conception .
	manualset3
115809	5	403511	5	NULL	NULL	0	NULL	increased probability	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison across cycles confirmed the hypothesis that higher ovarian steroid levels are associated with an increased probability of conception .
	manualset3
115810	6	403511	5	NULL	NULL	0	NULL	conception	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison across cycles confirmed the hypothesis that higher ovarian steroid levels are associated with an increased probability of conception .
	manualset3
115811	1	403512	5	NULL	NULL	0	NULL	PLA2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither PLA2 nor arachidonic acid alone will activate the cells ; it seems that agonist is essential .
	manualset3
115812	2	403512	5	NULL	NULL	0	NULL	arachidonic acid	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither PLA2 nor arachidonic acid alone will activate the cells ; it seems that agonist is essential .
	manualset3
115813	3	403512	5	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither PLA2 nor arachidonic acid alone will activate the cells ; it seems that agonist is essential .
	manualset3
115814	4	403512	5	NULL	NULL	0	NULL	agonist	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither PLA2 nor arachidonic acid alone will activate the cells ; it seems that agonist is essential .
	manualset3
115815	1	403513	5	NULL	NULL	0	NULL	SEB	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither SEB nor LPS produced lethal effects alone .
	manualset3
115816	2	403513	5	NULL	NULL	0	NULL	LPS	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither SEB nor LPS produced lethal effects alone .
	manualset3
115817	3	403513	5	NULL	NULL	0	NULL	lethal effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither SEB nor LPS produced lethal effects alone .
	manualset3
115818	1	403514	5	NULL	NULL	NULL	NULL	TAK-044 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Neither TAK-044 nor hydralazine affected plasma ET-1 concentration in this model .
	manualset3
115819	2	403514	5	NULL	NULL	0	NULL	hydralazine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither TAK-044 nor hydralazine affected plasma ET-1 concentration in this model .
	manualset3
115820	3	403514	5	NULL	NULL	0	NULL	plasma ET-1 concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither TAK-044 nor hydralazine affected plasma ET-1 concentration in this model .
	manualset3
115821	4	403514	5	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither TAK-044 nor hydralazine affected plasma ET-1 concentration in this model .
	manualset3
115822	1	403515	5	NULL	NULL	0	NULL	age	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither age nor fracture pattern is pathognomonic of abuse , but suspicion should remain high .
	manualset3
115823	2	403515	5	NULL	NULL	0	NULL	fracture pattern	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither age nor fracture pattern is pathognomonic of abuse , but suspicion should remain high .
	manualset3
115824	3	403515	5	NULL	NULL	0	NULL	abuse	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither age nor fracture pattern is pathognomonic of abuse , but suspicion should remain high .
	manualset3
115825	4	403515	5	NULL	NULL	0	NULL	suspicion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither age nor fracture pattern is pathognomonic of abuse , but suspicion should remain high .
	manualset3
115826	1	403516	5	NULL	NULL	0	NULL	diazepam	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither diazepam nor methylphenidate is without the potential for toxicity , which increases with dosage .
	manualset3
115827	2	403516	5	NULL	NULL	0	NULL	methylphenidate	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither diazepam nor methylphenidate is without the potential for toxicity , which increases with dosage .
	manualset3
115828	3	403516	5	NULL	NULL	0	NULL	potential	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither diazepam nor methylphenidate is without the potential for toxicity , which increases with dosage .
	manualset3
115829	4	403516	5	NULL	NULL	0	NULL	toxicity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither diazepam nor methylphenidate is without the potential for toxicity , which increases with dosage .
	manualset3
115830	5	403516	5	NULL	NULL	0	NULL	dosage	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither diazepam nor methylphenidate is without the potential for toxicity , which increases with dosage .
	manualset3
115845	1	403517	5	NULL	NULL	0	NULL	intracellular fluorescence 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither intracellular nor pericellular fluorescence was observed in the BT549 cells in the presence of cytochalasin B , suggesting that degradation occurred intracellularly and was dependent on endocytic uptake of substrate .
	manualset3
115846	2	403517	5	NULL	NULL	0	NULL	pericellular fluorescence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither intracellular nor pericellular fluorescence was observed in the BT549 cells in the presence of cytochalasin B , suggesting that degradation occurred intracellularly and was dependent on endocytic uptake of substrate .
	manualset3
115847	3	403517	5	NULL	NULL	0	NULL	BT549 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither intracellular nor pericellular fluorescence was observed in the BT549 cells in the presence of cytochalasin B , suggesting that degradation occurred intracellularly and was dependent on endocytic uptake of substrate .
	manualset3
115848	4	403517	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither intracellular nor pericellular fluorescence was observed in the BT549 cells in the presence of cytochalasin B , suggesting that degradation occurred intracellularly and was dependent on endocytic uptake of substrate .
	manualset3
115849	5	403517	5	NULL	NULL	0	NULL	cytochalasin B 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither intracellular nor pericellular fluorescence was observed in the BT549 cells in the presence of cytochalasin B , suggesting that degradation occurred intracellularly and was dependent on endocytic uptake of substrate .
	manualset3
115850	6	403517	5	NULL	NULL	0	NULL	degradation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither intracellular nor pericellular fluorescence was observed in the BT549 cells in the presence of cytochalasin B , suggesting that degradation occurred intracellularly and was dependent on endocytic uptake of substrate .
	manualset3
115851	7	403517	5	NULL	NULL	0	NULL	endocytic uptake	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither intracellular nor pericellular fluorescence was observed in the BT549 cells in the presence of cytochalasin B , suggesting that degradation occurred intracellularly and was dependent on endocytic uptake of substrate .
	manualset3
115852	8	403517	5	NULL	NULL	0	NULL	substrate 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither intracellular nor pericellular fluorescence was observed in the BT549 cells in the presence of cytochalasin B , suggesting that degradation occurred intracellularly and was dependent on endocytic uptake of substrate .
	manualset3
115854	1	403518	5	NULL	NULL	0	NULL	male NPSR1-deficient mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither male nor female NPSR1-deficient mice showed alterations of baseline locomotion , anxiety-like behavior , or corticosterone release after exposure to a forced swim test or methamphetamine challenge in an open-field .
	manualset3
115855	2	403518	5	NULL	NULL	0	NULL	female NPSR1-deficient mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither male nor female NPSR1-deficient mice showed alterations of baseline locomotion , anxiety-like behavior , or corticosterone release after exposure to a forced swim test or methamphetamine challenge in an open-field .
	manualset3
115856	3	403518	5	NULL	NULL	0	NULL	alterations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither male nor female NPSR1-deficient mice showed alterations of baseline locomotion , anxiety-like behavior , or corticosterone release after exposure to a forced swim test or methamphetamine challenge in an open-field .
	manualset3
115857	4	403518	5	NULL	NULL	0	NULL	baseline locomotion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither male nor female NPSR1-deficient mice showed alterations of baseline locomotion , anxiety-like behavior , or corticosterone release after exposure to a forced swim test or methamphetamine challenge in an open-field .
	manualset3
115858	5	403518	5	NULL	NULL	0	NULL	anxiety-like behavior	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither male nor female NPSR1-deficient mice showed alterations of baseline locomotion , anxiety-like behavior , or corticosterone release after exposure to a forced swim test or methamphetamine challenge in an open-field .
	manualset3
115859	6	403518	5	NULL	NULL	0	NULL	corticosterone release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither male nor female NPSR1-deficient mice showed alterations of baseline locomotion , anxiety-like behavior , or corticosterone release after exposure to a forced swim test or methamphetamine challenge in an open-field .
	manualset3
115861	7	403518	5	NULL	NULL	0	NULL	exposure 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither male nor female NPSR1-deficient mice showed alterations of baseline locomotion , anxiety-like behavior , or corticosterone release after exposure to a forced swim test or methamphetamine challenge in an open-field .
	manualset3
115862	8	403518	5	NULL	NULL	0	NULL	swim test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither male nor female NPSR1-deficient mice showed alterations of baseline locomotion , anxiety-like behavior , or corticosterone release after exposure to a forced swim test or methamphetamine challenge in an open-field .
	manualset3
115865	9	403518	5	NULL	NULL	0	NULL	methamphetamine challenge	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither male nor female NPSR1-deficient mice showed alterations of baseline locomotion , anxiety-like behavior , or corticosterone release after exposure to a forced swim test or methamphetamine challenge in an open-field .
	manualset3
115866	10	403518	5	NULL	NULL	0	NULL	open-field	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither male nor female NPSR1-deficient mice showed alterations of baseline locomotion , anxiety-like behavior , or corticosterone release after exposure to a forced swim test or methamphetamine challenge in an open-field .
	manualset3
115877	1	403519	5	NULL	NULL	0	NULL	ryanodine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither ryanodine nor BAY K 8644 altered the SI-induced changes in RMP .
	manualset3
115878	2	403519	5	NULL	NULL	0	NULL	BAY K 8644 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither ryanodine nor BAY K 8644 altered the SI-induced changes in RMP .
	manualset3
115879	3	403519	5	NULL	NULL	0	NULL	SI-induced changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither ryanodine nor BAY K 8644 altered the SI-induced changes in RMP .
	manualset3
115880	4	403519	5	NULL	NULL	0	NULL	RMP 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither ryanodine nor BAY K 8644 altered the SI-induced changes in RMP .
	manualset3
115881	1	403520	5	NULL	NULL	0	NULL	brain MRI	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither brain MRI and CT nor SPECT demonstrated any abnormalities .
	manualset3
115882	2	403520	5	NULL	NULL	0	NULL	brain CT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither brain MRI and CT nor SPECT demonstrated any abnormalities .
	manualset3
115883	3	403520	5	NULL	NULL	0	NULL	brain SPECT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither brain MRI and CT nor SPECT demonstrated any abnormalities .
	manualset3
115884	4	403520	5	NULL	NULL	0	NULL	abnormalities 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither brain MRI and CT nor SPECT demonstrated any abnormalities .
	manualset3
115885	1	403521	5	NULL	NULL	0	NULL	direct exposure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither direct exposure of cells to nor enrichment with 18 : 1 n-9 had any protective effect .
	manualset3
115886	2	403521	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither direct exposure of cells to nor enrichment with 18 : 1 n-9 had any protective effect .
	manualset3
115887	3	403521	5	NULL	NULL	0	NULL	enrichment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither direct exposure of cells to nor enrichment with 18 : 1 n-9 had any protective effect .
	manualset3
115888	4	403521	5	NULL	NULL	0	NULL	18 : 1 n-9	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither direct exposure of cells to nor enrichment with 18 : 1 n-9 had any protective effect .
	manualset3
115889	5	403521	5	NULL	NULL	0	NULL	protective effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither direct exposure of cells to nor enrichment with 18 : 1 n-9 had any protective effect .
	manualset3
115890	1	403522	5	NULL	NULL	0	NULL	elastic modulus 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither elastic modulus nor yield strength was significantly affected by the fatigue loading .
	manualset3
115891	2	403522	5	NULL	NULL	0	NULL	yield strength	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither elastic modulus nor yield strength was significantly affected by the fatigue loading .
	manualset3
115892	3	403522	5	NULL	NULL	0	NULL	fatigue loading	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither elastic modulus nor yield strength was significantly affected by the fatigue loading .
	manualset3
115893	1	403523	5	NULL	NULL	0	NULL	gastrointestinal tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither gastrointestinal tumor nor any signs of tuberous sclerosis were found .
	manualset3
115894	2	403523	5	NULL	NULL	0	NULL	signs 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither gastrointestinal tumor nor any signs of tuberous sclerosis were found .
	manualset3
115895	3	403523	5	NULL	NULL	0	NULL	tuberous sclerosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither gastrointestinal tumor nor any signs of tuberous sclerosis were found .
	manualset3
115896	1	403524	5	NULL	NULL	NULL	NULL	group 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Neither group substantially increased their overall coping responses , although men in the father-focused group significantly changed their coping efforts by seeking more social support , particularly getting information and emotional support from their partner 's physician .
	manualset3
115897	2	403524	5	NULL	NULL	0	NULL	overall coping responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither group substantially increased their overall coping responses , although men in the father-focused group significantly changed their coping efforts by seeking more social support , particularly getting information and emotional support from their partner 's physician .
	manualset3
115898	3	403524	5	NULL	NULL	0	NULL	men 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither group substantially increased their overall coping responses , although men in the father-focused group significantly changed their coping efforts by seeking more social support , particularly getting information and emotional support from their partner 's physician .
	manualset3
115899	4	403524	5	NULL	NULL	0	NULL	father-focused group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither group substantially increased their overall coping responses , although men in the father-focused group significantly changed their coping efforts by seeking more social support , particularly getting information and emotional support from their partner 's physician .
	manualset3
115900	5	403524	5	NULL	NULL	0	NULL	coping efforts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither group substantially increased their overall coping responses , although men in the father-focused group significantly changed their coping efforts by seeking more social support , particularly getting information and emotional support from their partner 's physician .
	manualset3
115901	6	403524	5	NULL	NULL	0	NULL	social support 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither group substantially increased their overall coping responses , although men in the father-focused group significantly changed their coping efforts by seeking more social support , particularly getting information and emotional support from their partner 's physician .
	manualset3
115902	7	403524	5	NULL	NULL	0	NULL	information 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither group substantially increased their overall coping responses , although men in the father-focused group significantly changed their coping efforts by seeking more social support , particularly getting information and emotional support from their partner 's physician .
	manualset3
115903	8	403524	5	NULL	NULL	0	NULL	emotional support 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither group substantially increased their overall coping responses , although men in the father-focused group significantly changed their coping efforts by seeking more social support , particularly getting information and emotional support from their partner 's physician .
	manualset3
115904	9	403524	5	NULL	NULL	0	NULL	partner 's physician	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither group substantially increased their overall coping responses , although men in the father-focused group significantly changed their coping efforts by seeking more social support , particularly getting information and emotional support from their partner 's physician .
	manualset3
115905	1	403525	5	NULL	NULL	NULL	NULL	hepatic concentration 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Neither hepatic concentration nor biliary excretion exhibited saturation over the dosage studied ( 6 -- 174 mg/kg ) .
	manualset3
115906	2	403525	5	NULL	NULL	0	NULL	biliary excretion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither hepatic concentration nor biliary excretion exhibited saturation over the dosage studied ( 6 -- 174 mg/kg ) .
	manualset3
115907	3	403525	5	NULL	NULL	0	NULL	saturation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither hepatic concentration nor biliary excretion exhibited saturation over the dosage studied ( 6 -- 174 mg/kg ) .
	manualset3
115908	4	403525	5	NULL	NULL	0	NULL	6 -- 174 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither hepatic concentration nor biliary excretion exhibited saturation over the dosage studied ( 6 -- 174 mg/kg ) .
	manualset3
115909	1	403526	5	NULL	NULL	0	NULL	neurological deterioration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither neurological deterioration nor deterioration of MRI abnormalities were observed during the clinical course .
	manualset3
115910	2	403526	5	NULL	NULL	0	NULL	deterioration 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither neurological deterioration nor deterioration of MRI abnormalities were observed during the clinical course .
	manualset3
115911	3	403526	5	NULL	NULL	0	NULL	MRI abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither neurological deterioration nor deterioration of MRI abnormalities were observed during the clinical course .
	manualset3
115912	4	403526	5	NULL	NULL	0	NULL	clinical course	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither neurological deterioration nor deterioration of MRI abnormalities were observed during the clinical course .
	manualset3
115914	1	403527	5	NULL	NULL	0	NULL	patient-related variables	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither patient-related variables ( age , gender , diabetes , hypertension , cigarette use , restenosis , previous myocardial infarction , and left ventricular function ) nor lesion characteristics ( length , ostial or bifurcation location , calcification , lesion classification , and coronary location ) were predictive of poor outcome .
	manualset3
115917	2	403527	5	NULL	NULL	NULL	NULL	age 	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Neither patient-related variables ( age , gender , diabetes , hypertension , cigarette use , restenosis , previous myocardial infarction , and left ventricular function ) nor lesion characteristics ( length , ostial or bifurcation location , calcification , lesion classification , and coronary location ) were predictive of poor outcome .
	manualset3
115918	3	403527	5	NULL	NULL	0	NULL	gender 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither patient-related variables ( age , gender , diabetes , hypertension , cigarette use , restenosis , previous myocardial infarction , and left ventricular function ) nor lesion characteristics ( length , ostial or bifurcation location , calcification , lesion classification , and coronary location ) were predictive of poor outcome .
	manualset3
115920	4	403527	5	NULL	NULL	0	NULL	diabetes 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither patient-related variables ( age , gender , diabetes , hypertension , cigarette use , restenosis , previous myocardial infarction , and left ventricular function ) nor lesion characteristics ( length , ostial or bifurcation location , calcification , lesion classification , and coronary location ) were predictive of poor outcome .
	manualset3
115921	5	403527	5	NULL	NULL	0	NULL	hypertension 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither patient-related variables ( age , gender , diabetes , hypertension , cigarette use , restenosis , previous myocardial infarction , and left ventricular function ) nor lesion characteristics ( length , ostial or bifurcation location , calcification , lesion classification , and coronary location ) were predictive of poor outcome .
	manualset3
115923	6	403527	5	NULL	NULL	0	NULL	cigarette use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither patient-related variables ( age , gender , diabetes , hypertension , cigarette use , restenosis , previous myocardial infarction , and left ventricular function ) nor lesion characteristics ( length , ostial or bifurcation location , calcification , lesion classification , and coronary location ) were predictive of poor outcome .
	manualset3
115924	7	403527	5	NULL	NULL	0	NULL	restenosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither patient-related variables ( age , gender , diabetes , hypertension , cigarette use , restenosis , previous myocardial infarction , and left ventricular function ) nor lesion characteristics ( length , ostial or bifurcation location , calcification , lesion classification , and coronary location ) were predictive of poor outcome .
	manualset3
115925	8	403527	5	NULL	NULL	0	NULL	previous myocardial infarction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither patient-related variables ( age , gender , diabetes , hypertension , cigarette use , restenosis , previous myocardial infarction , and left ventricular function ) nor lesion characteristics ( length , ostial or bifurcation location , calcification , lesion classification , and coronary location ) were predictive of poor outcome .
	manualset3
115926	9	403527	5	NULL	NULL	0	NULL	left ventricular function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither patient-related variables ( age , gender , diabetes , hypertension , cigarette use , restenosis , previous myocardial infarction , and left ventricular function ) nor lesion characteristics ( length , ostial or bifurcation location , calcification , lesion classification , and coronary location ) were predictive of poor outcome .
	manualset3
115927	10	403527	5	NULL	NULL	0	NULL	lesion characteristics 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither patient-related variables ( age , gender , diabetes , hypertension , cigarette use , restenosis , previous myocardial infarction , and left ventricular function ) nor lesion characteristics ( length , ostial or bifurcation location , calcification , lesion classification , and coronary location ) were predictive of poor outcome .
	manualset3
115928	11	403527	5	NULL	NULL	0	NULL	length 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither patient-related variables ( age , gender , diabetes , hypertension , cigarette use , restenosis , previous myocardial infarction , and left ventricular function ) nor lesion characteristics ( length , ostial or bifurcation location , calcification , lesion classification , and coronary location ) were predictive of poor outcome .
	manualset3
115929	12	403527	5	NULL	NULL	0	NULL	ostial or bifurcation location	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither patient-related variables ( age , gender , diabetes , hypertension , cigarette use , restenosis , previous myocardial infarction , and left ventricular function ) nor lesion characteristics ( length , ostial or bifurcation location , calcification , lesion classification , and coronary location ) were predictive of poor outcome .
	manualset3
115930	13	403527	5	NULL	NULL	0	NULL	calcification 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither patient-related variables ( age , gender , diabetes , hypertension , cigarette use , restenosis , previous myocardial infarction , and left ventricular function ) nor lesion characteristics ( length , ostial or bifurcation location , calcification , lesion classification , and coronary location ) were predictive of poor outcome .
	manualset3
115931	14	403527	5	NULL	NULL	0	NULL	lesion classification	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither patient-related variables ( age , gender , diabetes , hypertension , cigarette use , restenosis , previous myocardial infarction , and left ventricular function ) nor lesion characteristics ( length , ostial or bifurcation location , calcification , lesion classification , and coronary location ) were predictive of poor outcome .
	manualset3
115932	15	403527	5	NULL	NULL	0	NULL	coronary location	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither patient-related variables ( age , gender , diabetes , hypertension , cigarette use , restenosis , previous myocardial infarction , and left ventricular function ) nor lesion characteristics ( length , ostial or bifurcation location , calcification , lesion classification , and coronary location ) were predictive of poor outcome .
	manualset3
115933	16	403527	5	NULL	NULL	0	NULL	poor outcome	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither patient-related variables ( age , gender , diabetes , hypertension , cigarette use , restenosis , previous myocardial infarction , and left ventricular function ) nor lesion characteristics ( length , ostial or bifurcation location , calcification , lesion classification , and coronary location ) were predictive of poor outcome .
	manualset3
115934	1	403528	5	NULL	NULL	0	NULL	Neointima formation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neointima formation at 8 weeks was evidenced through collagen deposition and smooth muscle-like cells circumferential growth on the luminal surface without intimal hyperplasia or aneurysm formation .
	manualset3
115935	2	403528	5	NULL	NULL	0	NULL	8 weeks	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Neointima formation at 8 weeks was evidenced through collagen deposition and smooth muscle-like cells circumferential growth on the luminal surface without intimal hyperplasia or aneurysm formation .
	manualset3
115936	3	403528	5	NULL	NULL	0	NULL	collagen deposition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neointima formation at 8 weeks was evidenced through collagen deposition and smooth muscle-like cells circumferential growth on the luminal surface without intimal hyperplasia or aneurysm formation .
	manualset3
115937	4	403528	5	NULL	NULL	0	NULL	smooth muscle-like cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Neointima formation at 8 weeks was evidenced through collagen deposition and smooth muscle-like cells circumferential growth on the luminal surface without intimal hyperplasia or aneurysm formation .
	manualset3
115938	5	403528	5	NULL	NULL	0	NULL	circumferential growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neointima formation at 8 weeks was evidenced through collagen deposition and smooth muscle-like cells circumferential growth on the luminal surface without intimal hyperplasia or aneurysm formation .
	manualset3
115939	6	403528	5	NULL	NULL	0	NULL	luminal surface	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Neointima formation at 8 weeks was evidenced through collagen deposition and smooth muscle-like cells circumferential growth on the luminal surface without intimal hyperplasia or aneurysm formation .
	manualset3
115940	7	403528	5	NULL	NULL	0	NULL	intimal hyperplasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neointima formation at 8 weeks was evidenced through collagen deposition and smooth muscle-like cells circumferential growth on the luminal surface without intimal hyperplasia or aneurysm formation .
	manualset3
115941	8	403528	5	NULL	NULL	0	NULL	aneurysm formation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neointima formation at 8 weeks was evidenced through collagen deposition and smooth muscle-like cells circumferential growth on the luminal surface without intimal hyperplasia or aneurysm formation .
	manualset3
115942	1	403529	5	NULL	NULL	0	NULL	Neonatal binge ethanol treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonatal binge ethanol treatment significantly impaired acquisition of conditioning at both ages regardless of ISI , and deficits in the acquisition and expression of CRs were comparable across ISIs .
	manualset3
115943	2	403529	5	NULL	NULL	0	NULL	acquisition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonatal binge ethanol treatment significantly impaired acquisition of conditioning at both ages regardless of ISI , and deficits in the acquisition and expression of CRs were comparable across ISIs .
	manualset3
115944	3	403529	5	NULL	NULL	0	NULL	conditioning 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonatal binge ethanol treatment significantly impaired acquisition of conditioning at both ages regardless of ISI , and deficits in the acquisition and expression of CRs were comparable across ISIs .
	manualset3
115945	4	403529	5	NULL	NULL	0	NULL	both ages 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonatal binge ethanol treatment significantly impaired acquisition of conditioning at both ages regardless of ISI , and deficits in the acquisition and expression of CRs were comparable across ISIs .
	manualset3
115946	5	403529	5	NULL	NULL	0	NULL	ISI	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonatal binge ethanol treatment significantly impaired acquisition of conditioning at both ages regardless of ISI , and deficits in the acquisition and expression of CRs were comparable across ISIs .
	manualset3
115947	6	403529	5	NULL	NULL	0	NULL	deficits 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonatal binge ethanol treatment significantly impaired acquisition of conditioning at both ages regardless of ISI , and deficits in the acquisition and expression of CRs were comparable across ISIs .
	manualset3
115948	7	403529	5	NULL	NULL	0	NULL	acquisition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonatal binge ethanol treatment significantly impaired acquisition of conditioning at both ages regardless of ISI , and deficits in the acquisition and expression of CRs were comparable across ISIs .
	manualset3
115949	8	403529	5	NULL	NULL	0	NULL	expression 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonatal binge ethanol treatment significantly impaired acquisition of conditioning at both ages regardless of ISI , and deficits in the acquisition and expression of CRs were comparable across ISIs .
	manualset3
115950	9	403529	5	NULL	NULL	0	NULL	CRs	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonatal binge ethanol treatment significantly impaired acquisition of conditioning at both ages regardless of ISI , and deficits in the acquisition and expression of CRs were comparable across ISIs .
	manualset3
115951	10	403529	5	NULL	NULL	0	NULL	 ISIs	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonatal binge ethanol treatment significantly impaired acquisition of conditioning at both ages regardless of ISI , and deficits in the acquisition and expression of CRs were comparable across ISIs .
	manualset3
115952	1	403530	5	NULL	NULL	0	NULL	Neonatal capsaicin treatment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonatal capsaicin treatment modulates experience-dependent plasticity in the rat barrel cortex .
	manualset3
115953	2	403530	5	NULL	NULL	0	NULL	experience-dependent plasticity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonatal capsaicin treatment modulates experience-dependent plasticity in the rat barrel cortex .
	manualset3
115954	3	403530	5	NULL	NULL	0	NULL	rat barrel cortex	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonatal capsaicin treatment modulates experience-dependent plasticity in the rat barrel cortex .
	manualset3
115228	1	403531	13	NULL	NULL	0	NULL	Neonatal fluoxetine exposure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonatal fluoxetine exposure affects the action potential properties and dendritic development in cortical subplate neurons of rats .
	manualset3
115230	3	403531	13	NULL	NULL	NULL	NULL	action potential properties	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Neonatal fluoxetine exposure affects the action potential properties and dendritic development in cortical subplate neurons of rats .
	manualset3
115231	4	403531	13	NULL	NULL	0	NULL	dendritic development	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonatal fluoxetine exposure affects the action potential properties and dendritic development in cortical subplate neurons of rats .
	manualset3
115232	5	403531	13	NULL	NULL	0	NULL	cortical subplate neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonatal fluoxetine exposure affects the action potential properties and dendritic development in cortical subplate neurons of rats .
	manualset3
115233	6	403531	13	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonatal fluoxetine exposure affects the action potential properties and dendritic development in cortical subplate neurons of rats .
	manualset3
115234	1	403532	13	NULL	NULL	0	NULL	Neonatal parotitis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonatal parotitis is a rare condition .
	manualset3
115235	2	403532	13	NULL	NULL	0	NULL	condition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonatal parotitis is a rare condition .
	manualset3
115236	1	403533	13	NULL	NULL	0	NULL	Neonatal withdrawal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonatal withdrawal from methadone appeared to be more severe than from heroin , as judged by amount of medication required to control symptoms and duration of treatment .
	manualset3
115237	2	403533	13	NULL	NULL	0	NULL	methadone 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonatal withdrawal from methadone appeared to be more severe than from heroin , as judged by amount of medication required to control symptoms and duration of treatment .
	manualset3
115238	3	403533	13	NULL	NULL	0	NULL	heroin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonatal withdrawal from methadone appeared to be more severe than from heroin , as judged by amount of medication required to control symptoms and duration of treatment .
	manualset3
115239	4	403533	13	NULL	NULL	0	NULL	amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonatal withdrawal from methadone appeared to be more severe than from heroin , as judged by amount of medication required to control symptoms and duration of treatment .
	manualset3
115240	5	403533	13	NULL	NULL	0	NULL	medication	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonatal withdrawal from methadone appeared to be more severe than from heroin , as judged by amount of medication required to control symptoms and duration of treatment .
	manualset3
115241	6	403533	13	NULL	NULL	0	NULL	symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonatal withdrawal from methadone appeared to be more severe than from heroin , as judged by amount of medication required to control symptoms and duration of treatment .
	manualset3
115242	7	403533	13	NULL	NULL	0	NULL	duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonatal withdrawal from methadone appeared to be more severe than from heroin , as judged by amount of medication required to control symptoms and duration of treatment .
	manualset3
115243	8	403533	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonatal withdrawal from methadone appeared to be more severe than from heroin , as judged by amount of medication required to control symptoms and duration of treatment .
	manualset3
115246	1	403534	13	NULL	NULL	0	NULL	Neonates 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonates appear to be more sensitive to the cardiovascular effect of theophylline ; tachycardia occurs at plasma concentrations of 13 mg/L .
	manualset3
115248	2	403534	13	NULL	NULL	0	NULL	cardiovascular effect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonates appear to be more sensitive to the cardiovascular effect of theophylline ; tachycardia occurs at plasma concentrations of 13 mg/L .
	manualset3
115249	3	403534	13	NULL	NULL	0	NULL	theophylline	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonates appear to be more sensitive to the cardiovascular effect of theophylline ; tachycardia occurs at plasma concentrations of 13 mg/L .
	manualset3
115250	4	403534	13	NULL	NULL	0	NULL	tachycardia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonates appear to be more sensitive to the cardiovascular effect of theophylline ; tachycardia occurs at plasma concentrations of 13 mg/L .
	manualset3
115254	5	403534	13	NULL	NULL	0	NULL	plasma concentrations 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonates appear to be more sensitive to the cardiovascular effect of theophylline ; tachycardia occurs at plasma concentrations of 13 mg/L .
	manualset3
115256	6	403534	13	NULL	NULL	0	NULL	13 mg/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonates appear to be more sensitive to the cardiovascular effect of theophylline ; tachycardia occurs at plasma concentrations of 13 mg/L .
	manualset3
115258	1	403535	13	NULL	NULL	0	NULL	Neonates	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonates were shown to excrete much more unchanged lignocaine ( mean : 19.67 % ) compared with adults ( mean : 4.27 % ) and the proportion of the dose excreted as 4-hydroxyxylidine is considerably reduced in neonates ( neonate mean : 8.89 % ; adult mean : 63.78 % ) .
	manualset3
115259	2	403535	13	NULL	NULL	0	NULL	lignocaine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonates were shown to excrete much more unchanged lignocaine ( mean : 19.67 % ) compared with adults ( mean : 4.27 % ) and the proportion of the dose excreted as 4-hydroxyxylidine is considerably reduced in neonates ( neonate mean : 8.89 % ; adult mean : 63.78 % ) .
	manualset3
115260	3	403535	13	NULL	NULL	0	NULL	mean : 19.67 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonates were shown to excrete much more unchanged lignocaine ( mean : 19.67 % ) compared with adults ( mean : 4.27 % ) and the proportion of the dose excreted as 4-hydroxyxylidine is considerably reduced in neonates ( neonate mean : 8.89 % ; adult mean : 63.78 % ) .
	manualset3
115261	4	403535	13	NULL	NULL	0	NULL	adults 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonates were shown to excrete much more unchanged lignocaine ( mean : 19.67 % ) compared with adults ( mean : 4.27 % ) and the proportion of the dose excreted as 4-hydroxyxylidine is considerably reduced in neonates ( neonate mean : 8.89 % ; adult mean : 63.78 % ) .
	manualset3
115262	5	403535	13	NULL	NULL	0	NULL	mean : 4.27 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonates were shown to excrete much more unchanged lignocaine ( mean : 19.67 % ) compared with adults ( mean : 4.27 % ) and the proportion of the dose excreted as 4-hydroxyxylidine is considerably reduced in neonates ( neonate mean : 8.89 % ; adult mean : 63.78 % ) .
	manualset3
115263	6	403535	13	NULL	NULL	0	NULL	proportion	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonates were shown to excrete much more unchanged lignocaine ( mean : 19.67 % ) compared with adults ( mean : 4.27 % ) and the proportion of the dose excreted as 4-hydroxyxylidine is considerably reduced in neonates ( neonate mean : 8.89 % ; adult mean : 63.78 % ) .
	manualset3
115264	7	403535	13	NULL	NULL	0	NULL	dose	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonates were shown to excrete much more unchanged lignocaine ( mean : 19.67 % ) compared with adults ( mean : 4.27 % ) and the proportion of the dose excreted as 4-hydroxyxylidine is considerably reduced in neonates ( neonate mean : 8.89 % ; adult mean : 63.78 % ) .
	manualset3
115265	8	403535	13	NULL	NULL	0	NULL	4-hydroxyxylidine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonates were shown to excrete much more unchanged lignocaine ( mean : 19.67 % ) compared with adults ( mean : 4.27 % ) and the proportion of the dose excreted as 4-hydroxyxylidine is considerably reduced in neonates ( neonate mean : 8.89 % ; adult mean : 63.78 % ) .
	manualset3
115266	9	403535	13	NULL	NULL	0	NULL	neonates	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonates were shown to excrete much more unchanged lignocaine ( mean : 19.67 % ) compared with adults ( mean : 4.27 % ) and the proportion of the dose excreted as 4-hydroxyxylidine is considerably reduced in neonates ( neonate mean : 8.89 % ; adult mean : 63.78 % ) .
	manualset3
115267	10	403535	13	NULL	NULL	0	NULL	neonate mean : 8.89 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonates were shown to excrete much more unchanged lignocaine ( mean : 19.67 % ) compared with adults ( mean : 4.27 % ) and the proportion of the dose excreted as 4-hydroxyxylidine is considerably reduced in neonates ( neonate mean : 8.89 % ; adult mean : 63.78 % ) .
	manualset3
115268	11	403535	13	NULL	NULL	0	NULL	adult mean : 63.78 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonates were shown to excrete much more unchanged lignocaine ( mean : 19.67 % ) compared with adults ( mean : 4.27 % ) and the proportion of the dose excreted as 4-hydroxyxylidine is considerably reduced in neonates ( neonate mean : 8.89 % ; adult mean : 63.78 % ) .
	manualset3
115269	1	403536	13	NULL	NULL	0	NULL	Neonates 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonates with viral infection , bacterial colonization , or neonatal distress had normal or slightly increased levels .
	manualset3
115270	2	403536	13	NULL	NULL	0	NULL	viral infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonates with viral infection , bacterial colonization , or neonatal distress had normal or slightly increased levels .
	manualset3
115271	3	403536	13	NULL	NULL	0	NULL	bacterial colonization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonates with viral infection , bacterial colonization , or neonatal distress had normal or slightly increased levels .
	manualset3
115272	4	403536	13	NULL	NULL	0	NULL	neonatal distress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonates with viral infection , bacterial colonization , or neonatal distress had normal or slightly increased levels .
	manualset3
115273	5	403536	13	NULL	NULL	0	NULL	levels 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neonates with viral infection , bacterial colonization , or neonatal distress had normal or slightly increased levels .
	manualset3
115274	1	403537	13	NULL	NULL	0	NULL	Neoplastic transformation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neoplastic transformation of a human colonic epithelial cell line : in vitro evidence for the adenoma to carcinoma sequence .
	manualset3
115275	2	403537	13	NULL	NULL	0	NULL	human colonic epithelial cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Neoplastic transformation of a human colonic epithelial cell line : in vitro evidence for the adenoma to carcinoma sequence .
	manualset3
115276	3	403537	13	NULL	NULL	0	NULL	in vitro evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Neoplastic transformation of a human colonic epithelial cell line : in vitro evidence for the adenoma to carcinoma sequence .
	manualset3
115277	4	403537	13	NULL	NULL	NULL	NULL	adenoma to carcinoma sequence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Neoplastic transformation of a human colonic epithelial cell line : in vitro evidence for the adenoma to carcinoma sequence .
	manualset3
115278	1	403538	13	NULL	NULL	0	NULL	Neospora caninum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Neospora caninum is an apicomplexan parasite associated with abortion in cattle worldwide .
	manualset3
115279	2	403538	13	NULL	NULL	0	NULL	 apicomplexan parasite 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Neospora caninum is an apicomplexan parasite associated with abortion in cattle worldwide .
	manualset3
115280	3	403538	13	NULL	NULL	0	NULL	abortion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neospora caninum is an apicomplexan parasite associated with abortion in cattle worldwide .
	manualset3
115281	4	403538	13	NULL	NULL	0	NULL	cattle	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Neospora caninum is an apicomplexan parasite associated with abortion in cattle worldwide .
	manualset3
115282	1	403539	13	NULL	NULL	0	NULL	Neotran -- a new double-active pessary	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Neotran -- a new double-active pessary for the treatment of vaginitis .
	manualset3
115283	2	403539	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Neotran -- a new double-active pessary for the treatment of vaginitis .
	manualset3
115284	3	403539	13	NULL	NULL	0	NULL	vaginitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neotran -- a new double-active pessary for the treatment of vaginitis .
	manualset3
115285	1	403540	13	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison between the pathomorphological substrate and the X-ray morphometry of the shoulder joint was made with 482 arthroscopically treated patients .
	manualset3
115286	2	403540	13	NULL	NULL	NULL	NULL	pathomorphological substrate	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A comparison between the pathomorphological substrate and the X-ray morphometry of the shoulder joint was made with 482 arthroscopically treated patients .
	manualset3
115287	3	403540	13	NULL	NULL	0	NULL	X-ray morphometry	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison between the pathomorphological substrate and the X-ray morphometry of the shoulder joint was made with 482 arthroscopically treated patients .
	manualset3
115288	4	403540	13	NULL	NULL	0	NULL	shoulder joint	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison between the pathomorphological substrate and the X-ray morphometry of the shoulder joint was made with 482 arthroscopically treated patients .
	manualset3
115289	5	403540	13	NULL	NULL	0	NULL	482 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison between the pathomorphological substrate and the X-ray morphometry of the shoulder joint was made with 482 arthroscopically treated patients .
	manualset3
115290	6	403540	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison between the pathomorphological substrate and the X-ray morphometry of the shoulder joint was made with 482 arthroscopically treated patients .
	manualset3
115291	1	403541	13	NULL	NULL	0	NULL	Nepalese school-age children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nepalese school-age children reported relatively moderate levels of fears and limited use of coping strategies .
	manualset3
115292	2	403541	13	NULL	NULL	0	NULL	moderate levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nepalese school-age children reported relatively moderate levels of fears and limited use of coping strategies .
	manualset3
115293	3	403541	13	NULL	NULL	0	NULL	fears	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nepalese school-age children reported relatively moderate levels of fears and limited use of coping strategies .
	manualset3
115294	4	403541	13	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nepalese school-age children reported relatively moderate levels of fears and limited use of coping strategies .
	manualset3
115295	5	403541	13	NULL	NULL	0	NULL	coping strategies	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nepalese school-age children reported relatively moderate levels of fears and limited use of coping strategies .
	manualset3
115296	1	403542	13	NULL	NULL	0	NULL	Nephrolithiasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nephrolithiasis , Pyonephrosis and Impacted Urethral Calculus in a Boy Four Years of Age .
	manualset3
115297	2	403542	13	NULL	NULL	0	NULL	Pyonephrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nephrolithiasis , Pyonephrosis and Impacted Urethral Calculus in a Boy Four Years of Age .
	manualset3
115298	3	403542	13	NULL	NULL	0	NULL	Urethral Calculus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nephrolithiasis , Pyonephrosis and Impacted Urethral Calculus in a Boy Four Years of Age .
	manualset3
115299	4	403542	13	NULL	NULL	0	NULL	Boy	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Nephrolithiasis , Pyonephrosis and Impacted Urethral Calculus in a Boy Four Years of Age .
	manualset3
115300	5	403542	13	NULL	NULL	0	NULL	Four Years of Age	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Nephrolithiasis , Pyonephrosis and Impacted Urethral Calculus in a Boy Four Years of Age .
	manualset3
115301	1	403543	13	NULL	NULL	0	NULL	Nerve sheath myxoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nerve sheath myxoma of the oral cavity : case report and review .
	manualset3
115302	2	403543	13	NULL	NULL	0	NULL	oral cavity	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Nerve sheath myxoma of the oral cavity : case report and review .
	manualset3
115303	3	403543	13	NULL	NULL	0	NULL	case report 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Nerve sheath myxoma of the oral cavity : case report and review .
	manualset3
115304	4	403543	13	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Nerve sheath myxoma of the oral cavity : case report and review .
	manualset3
115305	1	403544	13	NULL	NULL	0	NULL	Net migration patterns	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Net migration patterns as well as the propensity to migrate by place of origin and destination are presented for different population groups according to birthplace .
	manualset3
115306	2	403544	13	NULL	NULL	0	NULL	propensity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Net migration patterns as well as the propensity to migrate by place of origin and destination are presented for different population groups according to birthplace .
	manualset3
115307	3	403544	13	NULL	NULL	0	NULL	place of origin	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Net migration patterns as well as the propensity to migrate by place of origin and destination are presented for different population groups according to birthplace .
	manualset3
115308	4	403544	13	NULL	NULL	0	NULL	destination 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Net migration patterns as well as the propensity to migrate by place of origin and destination are presented for different population groups according to birthplace .
	manualset3
115309	5	403544	13	NULL	NULL	0	NULL	different population groups 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Net migration patterns as well as the propensity to migrate by place of origin and destination are presented for different population groups according to birthplace .
	manualset3
115310	6	403544	13	NULL	NULL	0	NULL	birthplace	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Net migration patterns as well as the propensity to migrate by place of origin and destination are presented for different population groups according to birthplace .
	manualset3
115311	1	403545	13	NULL	NULL	0	NULL	Neu5Ac ( alpha2-6 ) Gal ( beta1-4 ) GlcNAc ( beta1-3 ) ( Gal ( alpha1-3 ) Gal ( beta1-4 ) ( Fuc ( alpha1-3 ) ) GlcNAc ( beta1-6 ) ) Gal ( beta1-4 ) Glc  	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Neu5Ac ( alpha2-6 ) Gal ( beta1-4 ) GlcNAc ( beta1-3 ) ( Gal ( alpha1-3 ) Gal ( beta1-4 ) ( Fuc ( alpha1-3 ) ) GlcNAc ( beta1-6 ) ) Gal ( beta1-4 ) Glc .
	manualset3
115312	1	403546	13	NULL	NULL	0	NULL	Neural excitability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neural excitability under these conditions could be sustained only until deoxygenation of the hemoglobin was complete .
	manualset3
115313	2	403546	13	NULL	NULL	0	NULL	conditions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neural excitability under these conditions could be sustained only until deoxygenation of the hemoglobin was complete .
	manualset3
115314	3	403546	13	NULL	NULL	0	NULL	deoxygenation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neural excitability under these conditions could be sustained only until deoxygenation of the hemoglobin was complete .
	manualset3
115315	4	403546	13	NULL	NULL	0	NULL	hemoglobin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Neural excitability under these conditions could be sustained only until deoxygenation of the hemoglobin was complete .
	manualset3
115316	1	403547	13	NULL	NULL	0	NULL	Neural networks 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neural networks were used for single feature combinations to optimise prediction of countershock success .
	manualset3
115317	2	403547	13	NULL	NULL	0	NULL	feature combinations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neural networks were used for single feature combinations to optimise prediction of countershock success .
	manualset3
115318	3	403547	13	NULL	NULL	0	NULL	prediction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neural networks were used for single feature combinations to optimise prediction of countershock success .
	manualset3
115319	4	403547	13	NULL	NULL	0	NULL	countershock success	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neural networks were used for single feature combinations to optimise prediction of countershock success .
	manualset3
115320	1	403548	13	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of attitudes toward the disabled in Ghana was made between 146 college students ( majoring in general education , special education administration and medicine ) and 128 non-students .
	manualset3
115321	2	403548	13	NULL	NULL	0	NULL	attitudes	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of attitudes toward the disabled in Ghana was made between 146 college students ( majoring in general education , special education administration and medicine ) and 128 non-students .
	manualset3
115322	3	403548	13	NULL	NULL	NULL	NULL	disabled 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A comparison of attitudes toward the disabled in Ghana was made between 146 college students ( majoring in general education , special education administration and medicine ) and 128 non-students .
	manualset3
115323	4	403548	13	NULL	NULL	0	NULL	Ghana	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of attitudes toward the disabled in Ghana was made between 146 college students ( majoring in general education , special education administration and medicine ) and 128 non-students .
	manualset3
115324	5	403548	13	NULL	NULL	0	NULL	146	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of attitudes toward the disabled in Ghana was made between 146 college students ( majoring in general education , special education administration and medicine ) and 128 non-students .
	manualset3
115325	6	403548	13	NULL	NULL	0	NULL	college students 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of attitudes toward the disabled in Ghana was made between 146 college students ( majoring in general education , special education administration and medicine ) and 128 non-students .
	manualset3
115326	7	403548	13	NULL	NULL	0	NULL	general education	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of attitudes toward the disabled in Ghana was made between 146 college students ( majoring in general education , special education administration and medicine ) and 128 non-students .
	manualset3
115327	8	403548	13	NULL	NULL	0	NULL	special education administration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of attitudes toward the disabled in Ghana was made between 146 college students ( majoring in general education , special education administration and medicine ) and 128 non-students .
	manualset3
115328	9	403548	13	NULL	NULL	0	NULL	medicine 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of attitudes toward the disabled in Ghana was made between 146 college students ( majoring in general education , special education administration and medicine ) and 128 non-students .
	manualset3
115329	10	403548	13	NULL	NULL	NULL	NULL	128	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A comparison of attitudes toward the disabled in Ghana was made between 146 college students ( majoring in general education , special education administration and medicine ) and 128 non-students .
	manualset3
115330	11	403548	13	NULL	NULL	0	NULL	non-students	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of attitudes toward the disabled in Ghana was made between 146 college students ( majoring in general education , special education administration and medicine ) and 128 non-students .
	manualset3
115331	1	403549	13	NULL	NULL	0	NULL	Neural stem cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Neural stem cells : the need for a proper orientation .
	manualset3
115332	2	403549	13	NULL	NULL	0	NULL	need	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neural stem cells : the need for a proper orientation .
	manualset3
115333	3	403549	13	NULL	NULL	0	NULL	orientation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neural stem cells : the need for a proper orientation .
	manualset3
115334	1	403550	13	NULL	NULL	0	NULL	Neurite-like processes 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurite-like processes are formed after addition of nerve growth factor .
	manualset3
115335	2	403550	13	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurite-like processes are formed after addition of nerve growth factor .
	manualset3
115336	3	403550	13	NULL	NULL	0	NULL	nerve growth factor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurite-like processes are formed after addition of nerve growth factor .
	manualset3
115337	1	403551	13	NULL	NULL	0	NULL	Neuroactive steroids 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroactive steroids : potential therapeutic use in neurological and psychiatric disorders .
	manualset3
115338	2	403551	13	NULL	NULL	0	NULL	therapeutic use	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroactive steroids : potential therapeutic use in neurological and psychiatric disorders .
	manualset3
115339	3	403551	13	NULL	NULL	0	NULL	neurological disorders 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroactive steroids : potential therapeutic use in neurological and psychiatric disorders .
	manualset3
115340	4	403551	13	NULL	NULL	0	NULL	psychiatric disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroactive steroids : potential therapeutic use in neurological and psychiatric disorders .
	manualset3
115341	1	403552	13	NULL	NULL	0	NULL	Neurobiology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurobiology , psychosomatic aspects and behavior therapy ) .
	manualset3
115342	2	403552	13	NULL	NULL	0	NULL	psychosomatic aspects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurobiology , psychosomatic aspects and behavior therapy ) .
	manualset3
115343	3	403552	13	NULL	NULL	0	NULL	behavior therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurobiology , psychosomatic aspects and behavior therapy ) .
	manualset3
115344	1	403553	13	NULL	NULL	0	NULL	Neuroblastoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroblastoma is a common solid tumor of childhood and advanced disease carries a poor prognosis despite intensive multimodality therapy .
	manualset3
115345	2	403553	13	NULL	NULL	0	NULL	solid tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroblastoma is a common solid tumor of childhood and advanced disease carries a poor prognosis despite intensive multimodality therapy .
	manualset3
115346	3	403553	13	NULL	NULL	0	NULL	childhood 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroblastoma is a common solid tumor of childhood and advanced disease carries a poor prognosis despite intensive multimodality therapy .
	manualset3
115347	4	403553	13	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroblastoma is a common solid tumor of childhood and advanced disease carries a poor prognosis despite intensive multimodality therapy .
	manualset3
115348	5	403553	13	NULL	NULL	0	NULL	prognosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroblastoma is a common solid tumor of childhood and advanced disease carries a poor prognosis despite intensive multimodality therapy .
	manualset3
115349	6	403553	13	NULL	NULL	0	NULL	intensive multimodality therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroblastoma is a common solid tumor of childhood and advanced disease carries a poor prognosis despite intensive multimodality therapy .
	manualset3
115350	1	403554	13	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of brain activation patterns during the two tasks with both fMRI and DSL indicated an involvement of the contralateral secondary somatosensory cortex in somatosensory categorization .
	manualset3
115352	2	403554	13	NULL	NULL	0	NULL	brain activation patterns 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of brain activation patterns during the two tasks with both fMRI and DSL indicated an involvement of the contralateral secondary somatosensory cortex in somatosensory categorization .
	manualset3
115353	3	403554	13	NULL	NULL	0	NULL	two tasks	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of brain activation patterns during the two tasks with both fMRI and DSL indicated an involvement of the contralateral secondary somatosensory cortex in somatosensory categorization .
	manualset3
115354	4	403554	13	NULL	NULL	0	NULL	fMRI	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of brain activation patterns during the two tasks with both fMRI and DSL indicated an involvement of the contralateral secondary somatosensory cortex in somatosensory categorization .
	manualset3
115355	5	403554	13	NULL	NULL	0	NULL	DSL	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of brain activation patterns during the two tasks with both fMRI and DSL indicated an involvement of the contralateral secondary somatosensory cortex in somatosensory categorization .
	manualset3
115356	6	403554	13	NULL	NULL	0	NULL	involvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of brain activation patterns during the two tasks with both fMRI and DSL indicated an involvement of the contralateral secondary somatosensory cortex in somatosensory categorization .
	manualset3
115357	7	403554	13	NULL	NULL	0	NULL	contralateral secondary somatosensory cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of brain activation patterns during the two tasks with both fMRI and DSL indicated an involvement of the contralateral secondary somatosensory cortex in somatosensory categorization .
	manualset3
115358	8	403554	13	NULL	NULL	0	NULL	somatosensory categorization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of brain activation patterns during the two tasks with both fMRI and DSL indicated an involvement of the contralateral secondary somatosensory cortex in somatosensory categorization .
	manualset3
115359	1	403555	13	NULL	NULL	0	NULL	Neurodegeneration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurodegeneration : diseases of the cytoskeleton ?
	manualset3
115360	2	403555	13	NULL	NULL	0	NULL	diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurodegeneration : diseases of the cytoskeleton ?
	manualset3
115361	3	403555	13	NULL	NULL	0	NULL	cytoskeleton	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurodegeneration : diseases of the cytoskeleton ?
	manualset3
115362	1	403556	13	NULL	NULL	0	NULL	Neuroelectric blocking factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroelectric blocking factors in human and animal sera evaluated using the isolated frog spinal cord .
	manualset3
115363	2	403556	13	NULL	NULL	0	NULL	human sera	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroelectric blocking factors in human and animal sera evaluated using the isolated frog spinal cord .
	manualset3
115364	3	403556	13	NULL	NULL	0	NULL	animal sera	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroelectric blocking factors in human and animal sera evaluated using the isolated frog spinal cord .
	manualset3
115365	4	403556	13	NULL	NULL	0	NULL	frog	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroelectric blocking factors in human and animal sera evaluated using the isolated frog spinal cord .
	manualset3
115366	5	403556	13	NULL	NULL	0	NULL	spinal cord	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroelectric blocking factors in human and animal sera evaluated using the isolated frog spinal cord .
	manualset3
115367	1	403557	13	NULL	NULL	0	NULL	Neuroendocrine responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroendocrine responses to cocaine do not exhibit sensitization following repeated cocaine exposure .
	manualset3
115368	2	403557	13	NULL	NULL	0	NULL	cocaine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroendocrine responses to cocaine do not exhibit sensitization following repeated cocaine exposure .
	manualset3
115369	3	403557	13	NULL	NULL	0	NULL	sensitization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroendocrine responses to cocaine do not exhibit sensitization following repeated cocaine exposure .
	manualset3
115370	4	403557	13	NULL	NULL	0	NULL	cocaine exposure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroendocrine responses to cocaine do not exhibit sensitization following repeated cocaine exposure .
	manualset3
115371	1	403558	13	NULL	NULL	0	NULL	Neuroendocrine responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroendocrine responses to serotonergic agents in alcoholics .
	manualset3
115372	2	403558	13	NULL	NULL	0	NULL	serotonergic agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroendocrine responses to serotonergic agents in alcoholics .
	manualset3
115373	3	403558	13	NULL	NULL	0	NULL	alcoholics 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroendocrine responses to serotonergic agents in alcoholics .
	manualset3
115374	1	403559	13	NULL	NULL	0	NULL	Neurogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurogenesis in the adult hippocampus is differentially influenced by the genetic background .
	manualset3
115375	2	403559	13	NULL	NULL	0	NULL	adult 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurogenesis in the adult hippocampus is differentially influenced by the genetic background .
	manualset3
115376	3	403559	13	NULL	NULL	0	NULL	hippocampus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurogenesis in the adult hippocampus is differentially influenced by the genetic background .
	manualset3
115377	4	403559	13	NULL	NULL	0	NULL	genetic background 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurogenesis in the adult hippocampus is differentially influenced by the genetic background .
	manualset3
115378	1	403560	13	NULL	NULL	0	NULL	Neuroimaging technologies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroimaging technologies have improved neurology and neurosurgery by providing tools to look inside the brain and investigate its functions and diseases .
	manualset3
115379	2	403560	13	NULL	NULL	0	NULL	neurology	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroimaging technologies have improved neurology and neurosurgery by providing tools to look inside the brain and investigate its functions and diseases .
	manualset3
115380	3	403560	13	NULL	NULL	0	NULL	neurosurgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroimaging technologies have improved neurology and neurosurgery by providing tools to look inside the brain and investigate its functions and diseases .
	manualset3
115381	4	403560	13	NULL	NULL	0	NULL	tools	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroimaging technologies have improved neurology and neurosurgery by providing tools to look inside the brain and investigate its functions and diseases .
	manualset3
115382	5	403560	13	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroimaging technologies have improved neurology and neurosurgery by providing tools to look inside the brain and investigate its functions and diseases .
	manualset3
115383	6	403560	13	NULL	NULL	0	NULL	functions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroimaging technologies have improved neurology and neurosurgery by providing tools to look inside the brain and investigate its functions and diseases .
	manualset3
115384	7	403560	13	NULL	NULL	0	NULL	diseases 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroimaging technologies have improved neurology and neurosurgery by providing tools to look inside the brain and investigate its functions and diseases .
	manualset3
115447	1	403561	13	NULL	NULL	0	NULL	Neurologic complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurologic complications are associated with increased disability , longer hospital stay , and increased mortality .
	manualset3
115448	2	403561	13	NULL	NULL	0	NULL	disability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurologic complications are associated with increased disability , longer hospital stay , and increased mortality .
	manualset3
115449	3	403561	13	NULL	NULL	0	NULL	hospital stay	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurologic complications are associated with increased disability , longer hospital stay , and increased mortality .
	manualset3
115450	4	403561	13	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurologic complications are associated with increased disability , longer hospital stay , and increased mortality .
	manualset3
115451	1	403562	13	NULL	NULL	0	NULL	Neurological diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurological diseases , such as multiple sclerosis ( MS ) , Sjgren-Larsson syndrome , Reye 's syndrome , and Refsum 's syndrome ( herediopathica atactica polyneuroformis ) , and many others afflict millions of persons yearly and have no successful treatment available .
	manualset3
115452	2	403562	13	NULL	NULL	0	NULL	multiple sclerosis ( MS )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurological diseases , such as multiple sclerosis ( MS ) , Sjgren-Larsson syndrome , Reye 's syndrome , and Refsum 's syndrome ( herediopathica atactica polyneuroformis ) , and many others afflict millions of persons yearly and have no successful treatment available .
	manualset3
115453	3	403562	13	NULL	NULL	0	NULL	Sjgren-Larsson syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurological diseases , such as multiple sclerosis ( MS ) , Sjgren-Larsson syndrome , Reye 's syndrome , and Refsum 's syndrome ( herediopathica atactica polyneuroformis ) , and many others afflict millions of persons yearly and have no successful treatment available .
	manualset3
115454	4	403562	13	NULL	NULL	0	NULL	Reye 's syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurological diseases , such as multiple sclerosis ( MS ) , Sjgren-Larsson syndrome , Reye 's syndrome , and Refsum 's syndrome ( herediopathica atactica polyneuroformis ) , and many others afflict millions of persons yearly and have no successful treatment available .
	manualset3
115455	5	403562	13	NULL	NULL	0	NULL	Refsum 's syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurological diseases , such as multiple sclerosis ( MS ) , Sjgren-Larsson syndrome , Reye 's syndrome , and Refsum 's syndrome ( herediopathica atactica polyneuroformis ) , and many others afflict millions of persons yearly and have no successful treatment available .
	manualset3
115456	6	403562	13	NULL	NULL	0	NULL	herediopathica atactica polyneuroformis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurological diseases , such as multiple sclerosis ( MS ) , Sjgren-Larsson syndrome , Reye 's syndrome , and Refsum 's syndrome ( herediopathica atactica polyneuroformis ) , and many others afflict millions of persons yearly and have no successful treatment available .
	manualset3
115457	7	403562	13	NULL	NULL	0	NULL	many others	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurological diseases , such as multiple sclerosis ( MS ) , Sjgren-Larsson syndrome , Reye 's syndrome , and Refsum 's syndrome ( herediopathica atactica polyneuroformis ) , and many others afflict millions of persons yearly and have no successful treatment available .
	manualset3
115458	8	403562	13	NULL	NULL	0	NULL	millions	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurological diseases , such as multiple sclerosis ( MS ) , Sjgren-Larsson syndrome , Reye 's syndrome , and Refsum 's syndrome ( herediopathica atactica polyneuroformis ) , and many others afflict millions of persons yearly and have no successful treatment available .
	manualset3
115459	9	403562	13	NULL	NULL	0	NULL	persons	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurological diseases , such as multiple sclerosis ( MS ) , Sjgren-Larsson syndrome , Reye 's syndrome , and Refsum 's syndrome ( herediopathica atactica polyneuroformis ) , and many others afflict millions of persons yearly and have no successful treatment available .
	manualset3
115460	10	403562	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurological diseases , such as multiple sclerosis ( MS ) , Sjgren-Larsson syndrome , Reye 's syndrome , and Refsum 's syndrome ( herediopathica atactica polyneuroformis ) , and many others afflict millions of persons yearly and have no successful treatment available .
	manualset3
115461	1	403563	13	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of canal centering ability of four instrumentation techniques .
	manualset3
115462	2	403563	13	NULL	NULL	0	NULL	canal centering ability	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of canal centering ability of four instrumentation techniques .
	manualset3
115463	3	403563	13	NULL	NULL	0	NULL	four instrumentation techniques	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of canal centering ability of four instrumentation techniques .
	manualset3
115464	1	403564	13	NULL	NULL	0	NULL	Neurological disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurological disorders and the potential role for stem cells as a therapy .
	manualset3
115465	2	403564	13	NULL	NULL	0	NULL	potential role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurological disorders and the potential role for stem cells as a therapy .
	manualset3
115466	3	403564	13	NULL	NULL	0	NULL	stem cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurological disorders and the potential role for stem cells as a therapy .
	manualset3
115467	4	403564	13	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurological disorders and the potential role for stem cells as a therapy .
	manualset3
115468	1	403565	13	NULL	NULL	0	NULL	Neurological examination 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurological examination revealed that the patient was suffering from right pyramidal sign as well as left deep sensory disturbance without apparent impairment of cranial nerves or nystagmus .
	manualset3
115469	2	403565	13	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurological examination revealed that the patient was suffering from right pyramidal sign as well as left deep sensory disturbance without apparent impairment of cranial nerves or nystagmus .
	manualset3
115470	3	403565	13	NULL	NULL	0	NULL	right pyramidal sign	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurological examination revealed that the patient was suffering from right pyramidal sign as well as left deep sensory disturbance without apparent impairment of cranial nerves or nystagmus .
	manualset3
115471	4	403565	13	NULL	NULL	0	NULL	left deep sensory disturbance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurological examination revealed that the patient was suffering from right pyramidal sign as well as left deep sensory disturbance without apparent impairment of cranial nerves or nystagmus .
	manualset3
115472	5	403565	13	NULL	NULL	0	NULL	impairment of cranial nerves	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurological examination revealed that the patient was suffering from right pyramidal sign as well as left deep sensory disturbance without apparent impairment of cranial nerves or nystagmus .
	manualset3
115473	6	403565	13	NULL	NULL	0	NULL	nystagmus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurological examination revealed that the patient was suffering from right pyramidal sign as well as left deep sensory disturbance without apparent impairment of cranial nerves or nystagmus .
	manualset3
115512	1	403566	13	NULL	NULL	0	NULL	Neurological symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurological symptoms , primarily due to involvement of the foramina , have been reported but are not common .
	manualset3
115513	2	403566	13	NULL	NULL	0	NULL	involvement 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurological symptoms , primarily due to involvement of the foramina , have been reported but are not common .
	manualset3
115516	3	403566	13	NULL	NULL	0	NULL	foramina	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurological symptoms , primarily due to involvement of the foramina , have been reported but are not common .
	manualset3
115518	1	403567	13	NULL	NULL	0	NULL	Neurological symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurological symptoms related to gonadotropin-releasing hormone agonist , low estrogen , or ?
	manualset3
115519	2	403567	13	NULL	NULL	0	NULL	gonadotropin-releasing hormone agonist	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurological symptoms related to gonadotropin-releasing hormone agonist , low estrogen , or ?
	manualset3
115520	3	403567	13	NULL	NULL	0	NULL	low estrogen	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurological symptoms related to gonadotropin-releasing hormone agonist , low estrogen , or ?
	manualset3
115522	1	403568	13	NULL	NULL	0	NULL	Neuromodulation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuromodulation independently determines correlated channel expression and conductance levels in motor neurons of the stomatogastric ganglion .
	manualset3
115528	2	403568	13	NULL	NULL	0	NULL	channel expression 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuromodulation independently determines correlated channel expression and conductance levels in motor neurons of the stomatogastric ganglion .
	manualset3
115529	3	403568	13	NULL	NULL	0	NULL	conductance levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuromodulation independently determines correlated channel expression and conductance levels in motor neurons of the stomatogastric ganglion .
	manualset3
115530	4	403568	13	NULL	NULL	0	NULL	motor neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuromodulation independently determines correlated channel expression and conductance levels in motor neurons of the stomatogastric ganglion .
	manualset3
115532	5	403568	13	NULL	NULL	0	NULL	stomatogastric ganglion	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuromodulation independently determines correlated channel expression and conductance levels in motor neurons of the stomatogastric ganglion .
	manualset3
115537	1	403569	13	NULL	NULL	0	NULL	Neuromuscular and vascular hamartoma ( NMVH )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuromuscular and vascular hamartoma ( NMVH ) is a very rare stricturing condition of the small intestine , occurring focally and causing recurrent obstructive symptoms or occult chronic gastrointestinal bleeding .
	manualset3
115539	2	403569	13	NULL	NULL	0	NULL	stricturing condition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuromuscular and vascular hamartoma ( NMVH ) is a very rare stricturing condition of the small intestine , occurring focally and causing recurrent obstructive symptoms or occult chronic gastrointestinal bleeding .
	manualset3
115540	3	403569	13	NULL	NULL	0	NULL	small intestine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuromuscular and vascular hamartoma ( NMVH ) is a very rare stricturing condition of the small intestine , occurring focally and causing recurrent obstructive symptoms or occult chronic gastrointestinal bleeding .
	manualset3
115541	4	403569	13	NULL	NULL	0	NULL	obstructive symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuromuscular and vascular hamartoma ( NMVH ) is a very rare stricturing condition of the small intestine , occurring focally and causing recurrent obstructive symptoms or occult chronic gastrointestinal bleeding .
	manualset3
115542	5	403569	13	NULL	NULL	0	NULL	occult chronic gastrointestinal bleeding 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuromuscular and vascular hamartoma ( NMVH ) is a very rare stricturing condition of the small intestine , occurring focally and causing recurrent obstructive symptoms or occult chronic gastrointestinal bleeding .
	manualset3
115546	1	403570	13	NULL	NULL	NULL	NULL	Neuronal activity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Neuronal activity in vitro and the in vivo reality : the role of energy homeostasis .
	manualset3
115548	2	403570	13	NULL	NULL	NULL	NULL	role	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Neuronal activity in vitro and the in vivo reality : the role of energy homeostasis .
	manualset3
115550	3	403570	13	NULL	NULL	0	NULL	energy homeostasis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuronal activity in vitro and the in vivo reality : the role of energy homeostasis .
	manualset3
115554	1	403571	13	NULL	NULL	0	NULL	Neuronal activity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuronal activity in human right lateral temporal cortex related to visuospatial memory and perception .
	manualset3
115555	2	403571	13	NULL	NULL	0	NULL	human right lateral temporal cortex 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuronal activity in human right lateral temporal cortex related to visuospatial memory and perception .
	manualset3
115556	3	403571	13	NULL	NULL	0	NULL	visuospatial memory	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuronal activity in human right lateral temporal cortex related to visuospatial memory and perception .
	manualset3
115557	4	403571	13	NULL	NULL	0	NULL	perception	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuronal activity in human right lateral temporal cortex related to visuospatial memory and perception .
	manualset3
115558	1	403572	13	NULL	NULL	0	NULL	Neuronal activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuronal activity of 58 cells in the lateral nucleus of the amygdala of freely moving cats was studied across stages of sleep-wakefulness .
	manualset3
115559	2	403572	13	NULL	NULL	0	NULL	58 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuronal activity of 58 cells in the lateral nucleus of the amygdala of freely moving cats was studied across stages of sleep-wakefulness .
	manualset3
115560	3	403572	13	NULL	NULL	0	NULL	lateral nucleus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuronal activity of 58 cells in the lateral nucleus of the amygdala of freely moving cats was studied across stages of sleep-wakefulness .
	manualset3
115561	4	403572	13	NULL	NULL	0	NULL	amygdala	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuronal activity of 58 cells in the lateral nucleus of the amygdala of freely moving cats was studied across stages of sleep-wakefulness .
	manualset3
115562	5	403572	13	NULL	NULL	0	NULL	cats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuronal activity of 58 cells in the lateral nucleus of the amygdala of freely moving cats was studied across stages of sleep-wakefulness .
	manualset3
115563	6	403572	13	NULL	NULL	0	NULL	stages of sleep-wakefulness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuronal activity of 58 cells in the lateral nucleus of the amygdala of freely moving cats was studied across stages of sleep-wakefulness .
	manualset3
115564	1	403573	13	NULL	NULL	NULL	NULL	comparison	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A comparison of civilian ( National Confidential Enquiry into Patient Outcome and Death ) trauma standards with current practice in a deployed field hospital in Afghanistan .
	manualset3
115565	2	403573	13	NULL	NULL	NULL	NULL	National Confidential Enquiry into Patient Outcome and Death	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A comparison of civilian ( National Confidential Enquiry into Patient Outcome and Death ) trauma standards with current practice in a deployed field hospital in Afghanistan .
	manualset3
115568	5	403573	13	NULL	NULL	0	NULL	trauma standards	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of civilian ( National Confidential Enquiry into Patient Outcome and Death ) trauma standards with current practice in a deployed field hospital in Afghanistan .
	manualset3
115569	6	403573	13	NULL	NULL	0	NULL	practice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of civilian ( National Confidential Enquiry into Patient Outcome and Death ) trauma standards with current practice in a deployed field hospital in Afghanistan .
	manualset3
115570	7	403573	13	NULL	NULL	0	NULL	field hospital 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of civilian ( National Confidential Enquiry into Patient Outcome and Death ) trauma standards with current practice in a deployed field hospital in Afghanistan .
	manualset3
115571	8	403573	13	NULL	NULL	0	NULL	Afghanistan	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of civilian ( National Confidential Enquiry into Patient Outcome and Death ) trauma standards with current practice in a deployed field hospital in Afghanistan .
	manualset3
115575	1	403574	13	NULL	NULL	0	NULL	Neuronal damage 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuronal damage was extensive in the piriform and entorhinal cortices , the hippocampal CA3 area and the polymorphic layer of the dentate gyrus , basal amygdala , mediodorsal thalamus and anterior olfactory nuclei .
	manualset3
115576	2	403574	13	NULL	NULL	0	NULL	piriform 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuronal damage was extensive in the piriform and entorhinal cortices , the hippocampal CA3 area and the polymorphic layer of the dentate gyrus , basal amygdala , mediodorsal thalamus and anterior olfactory nuclei .
	manualset3
115578	3	403574	13	NULL	NULL	0	NULL	entorhinal cortices 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuronal damage was extensive in the piriform and entorhinal cortices , the hippocampal CA3 area and the polymorphic layer of the dentate gyrus , basal amygdala , mediodorsal thalamus and anterior olfactory nuclei .
	manualset3
115579	4	403574	13	NULL	NULL	0	NULL	hippocampal CA3 area	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuronal damage was extensive in the piriform and entorhinal cortices , the hippocampal CA3 area and the polymorphic layer of the dentate gyrus , basal amygdala , mediodorsal thalamus and anterior olfactory nuclei .
	manualset3
115581	5	403574	13	NULL	NULL	0	NULL	polymorphic layer 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuronal damage was extensive in the piriform and entorhinal cortices , the hippocampal CA3 area and the polymorphic layer of the dentate gyrus , basal amygdala , mediodorsal thalamus and anterior olfactory nuclei .
	manualset3
115582	6	403574	13	NULL	NULL	0	NULL	dentate gyrus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuronal damage was extensive in the piriform and entorhinal cortices , the hippocampal CA3 area and the polymorphic layer of the dentate gyrus , basal amygdala , mediodorsal thalamus and anterior olfactory nuclei .
	manualset3
115584	7	403574	13	NULL	NULL	0	NULL	basal amygdala	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuronal damage was extensive in the piriform and entorhinal cortices , the hippocampal CA3 area and the polymorphic layer of the dentate gyrus , basal amygdala , mediodorsal thalamus and anterior olfactory nuclei .
	manualset3
115585	8	403574	13	NULL	NULL	0	NULL	mediodorsal thalamus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuronal damage was extensive in the piriform and entorhinal cortices , the hippocampal CA3 area and the polymorphic layer of the dentate gyrus , basal amygdala , mediodorsal thalamus and anterior olfactory nuclei .
	manualset3
115586	9	403574	13	NULL	NULL	0	NULL	anterior olfactory nuclei	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuronal damage was extensive in the piriform and entorhinal cortices , the hippocampal CA3 area and the polymorphic layer of the dentate gyrus , basal amygdala , mediodorsal thalamus and anterior olfactory nuclei .
	manualset3
115587	1	403575	13	NULL	NULL	0	NULL	Neurons 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurons of compact and dorsal parts of substantia nigra and scanty amygdala neurons project on the dorsal zone .
	manualset3
115589	2	403575	13	NULL	NULL	0	NULL	dorsal parts of substantia nigra	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurons of compact and dorsal parts of substantia nigra and scanty amygdala neurons project on the dorsal zone .
	manualset3
115592	3	403575	13	NULL	NULL	0	NULL	amygdala neurons 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurons of compact and dorsal parts of substantia nigra and scanty amygdala neurons project on the dorsal zone .
	manualset3
115593	4	403575	13	NULL	NULL	0	NULL	dorsal zone 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurons of compact and dorsal parts of substantia nigra and scanty amygdala neurons project on the dorsal zone .
	manualset3
115595	1	403576	13	NULL	NULL	0	NULL	Neurons 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurons of the supramammillary nucleus are known to fire phase-locked to hippocampal theta rhythm .
	manualset3
115596	2	403576	13	NULL	NULL	0	NULL	supramammillary nucleus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurons of the supramammillary nucleus are known to fire phase-locked to hippocampal theta rhythm .
	manualset3
115598	3	403576	13	NULL	NULL	0	NULL	 hippocampal theta rhythm	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurons of the supramammillary nucleus are known to fire phase-locked to hippocampal theta rhythm .
	manualset3
115601	1	403577	13	NULL	NULL	0	NULL	Neuropathic pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathic pain is defined as pain arising as a direct consequence of a lesion or disease affecting the somatosensory system either at peripheral or central level .
	manualset3
115602	2	403577	13	NULL	NULL	0	NULL	pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathic pain is defined as pain arising as a direct consequence of a lesion or disease affecting the somatosensory system either at peripheral or central level .
	manualset3
115603	3	403577	13	NULL	NULL	0	NULL	consequence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathic pain is defined as pain arising as a direct consequence of a lesion or disease affecting the somatosensory system either at peripheral or central level .
	manualset3
115605	4	403577	13	NULL	NULL	0	NULL	lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathic pain is defined as pain arising as a direct consequence of a lesion or disease affecting the somatosensory system either at peripheral or central level .
	manualset3
115606	5	403577	13	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathic pain is defined as pain arising as a direct consequence of a lesion or disease affecting the somatosensory system either at peripheral or central level .
	manualset3
115607	6	403577	13	NULL	NULL	0	NULL	somatosensory system 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathic pain is defined as pain arising as a direct consequence of a lesion or disease affecting the somatosensory system either at peripheral or central level .
	manualset3
115609	7	403577	13	NULL	NULL	0	NULL	peripheral level 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathic pain is defined as pain arising as a direct consequence of a lesion or disease affecting the somatosensory system either at peripheral or central level .
	manualset3
115610	8	403577	13	NULL	NULL	0	NULL	central level	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathic pain is defined as pain arising as a direct consequence of a lesion or disease affecting the somatosensory system either at peripheral or central level .
	manualset3
115612	1	403578	13	NULL	NULL	0	NULL	Neuropathic pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathic pain is responsible for a significant amount of the morbidity associated with generalized and focal peripheral neuropathies in diabetes .
	manualset3
115614	2	403578	13	NULL	NULL	0	NULL	significant amount	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathic pain is responsible for a significant amount of the morbidity associated with generalized and focal peripheral neuropathies in diabetes .
	manualset3
115616	3	403578	13	NULL	NULL	0	NULL	morbidity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathic pain is responsible for a significant amount of the morbidity associated with generalized and focal peripheral neuropathies in diabetes .
	manualset3
115617	4	403578	13	NULL	NULL	0	NULL	generalized neuropathies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathic pain is responsible for a significant amount of the morbidity associated with generalized and focal peripheral neuropathies in diabetes .
	manualset3
115618	5	403578	13	NULL	NULL	0	NULL	focal peripheral neuropathies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathic pain is responsible for a significant amount of the morbidity associated with generalized and focal peripheral neuropathies in diabetes .
	manualset3
115619	6	403578	13	NULL	NULL	0	NULL	diabetes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathic pain is responsible for a significant amount of the morbidity associated with generalized and focal peripheral neuropathies in diabetes .
	manualset3
115620	1	403579	13	NULL	NULL	0	NULL	Neuropathological assessment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathological assessment showed that 71 ( 84 % ) victims had sustained cerebral contusions , 49 ( 58 % ) had diffuse axonal injury ( DAI ) , 57 ( 67 % ) , had ischemic brain damage ( IBD ) , 58 ( 68 % ) had symmetrical ventricular enlargement , and in 47 ( 55 % ) intracranial pressure ( ICP ) had been increased .
	manualset3
115621	2	403579	13	NULL	NULL	0	NULL	71 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathological assessment showed that 71 ( 84 % ) victims had sustained cerebral contusions , 49 ( 58 % ) had diffuse axonal injury ( DAI ) , 57 ( 67 % ) , had ischemic brain damage ( IBD ) , 58 ( 68 % ) had symmetrical ventricular enlargement , and in 47 ( 55 % ) intracranial pressure ( ICP ) had been increased .
	manualset3
115622	3	403579	13	NULL	NULL	0	NULL	84 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathological assessment showed that 71 ( 84 % ) victims had sustained cerebral contusions , 49 ( 58 % ) had diffuse axonal injury ( DAI ) , 57 ( 67 % ) , had ischemic brain damage ( IBD ) , 58 ( 68 % ) had symmetrical ventricular enlargement , and in 47 ( 55 % ) intracranial pressure ( ICP ) had been increased .
	manualset3
115623	4	403579	13	NULL	NULL	0	NULL	victims	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathological assessment showed that 71 ( 84 % ) victims had sustained cerebral contusions , 49 ( 58 % ) had diffuse axonal injury ( DAI ) , 57 ( 67 % ) , had ischemic brain damage ( IBD ) , 58 ( 68 % ) had symmetrical ventricular enlargement , and in 47 ( 55 % ) intracranial pressure ( ICP ) had been increased .
	manualset3
115624	5	403579	13	NULL	NULL	0	NULL	cerebral contusions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathological assessment showed that 71 ( 84 % ) victims had sustained cerebral contusions , 49 ( 58 % ) had diffuse axonal injury ( DAI ) , 57 ( 67 % ) , had ischemic brain damage ( IBD ) , 58 ( 68 % ) had symmetrical ventricular enlargement , and in 47 ( 55 % ) intracranial pressure ( ICP ) had been increased .
	manualset3
115625	6	403579	13	NULL	NULL	0	NULL	49	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathological assessment showed that 71 ( 84 % ) victims had sustained cerebral contusions , 49 ( 58 % ) had diffuse axonal injury ( DAI ) , 57 ( 67 % ) , had ischemic brain damage ( IBD ) , 58 ( 68 % ) had symmetrical ventricular enlargement , and in 47 ( 55 % ) intracranial pressure ( ICP ) had been increased .
	manualset3
115626	7	403579	13	NULL	NULL	0	NULL	58 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathological assessment showed that 71 ( 84 % ) victims had sustained cerebral contusions , 49 ( 58 % ) had diffuse axonal injury ( DAI ) , 57 ( 67 % ) , had ischemic brain damage ( IBD ) , 58 ( 68 % ) had symmetrical ventricular enlargement , and in 47 ( 55 % ) intracranial pressure ( ICP ) had been increased .
	manualset3
115627	8	403579	13	NULL	NULL	0	NULL	diffuse axonal injury ( DAI )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathological assessment showed that 71 ( 84 % ) victims had sustained cerebral contusions , 49 ( 58 % ) had diffuse axonal injury ( DAI ) , 57 ( 67 % ) , had ischemic brain damage ( IBD ) , 58 ( 68 % ) had symmetrical ventricular enlargement , and in 47 ( 55 % ) intracranial pressure ( ICP ) had been increased .
	manualset3
115628	9	403579	13	NULL	NULL	0	NULL	57	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathological assessment showed that 71 ( 84 % ) victims had sustained cerebral contusions , 49 ( 58 % ) had diffuse axonal injury ( DAI ) , 57 ( 67 % ) , had ischemic brain damage ( IBD ) , 58 ( 68 % ) had symmetrical ventricular enlargement , and in 47 ( 55 % ) intracranial pressure ( ICP ) had been increased .
	manualset3
115629	10	403579	13	NULL	NULL	0	NULL	67 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathological assessment showed that 71 ( 84 % ) victims had sustained cerebral contusions , 49 ( 58 % ) had diffuse axonal injury ( DAI ) , 57 ( 67 % ) , had ischemic brain damage ( IBD ) , 58 ( 68 % ) had symmetrical ventricular enlargement , and in 47 ( 55 % ) intracranial pressure ( ICP ) had been increased .
	manualset3
115630	11	403579	13	NULL	NULL	0	NULL	 ischemic brain damage ( IBD ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathological assessment showed that 71 ( 84 % ) victims had sustained cerebral contusions , 49 ( 58 % ) had diffuse axonal injury ( DAI ) , 57 ( 67 % ) , had ischemic brain damage ( IBD ) , 58 ( 68 % ) had symmetrical ventricular enlargement , and in 47 ( 55 % ) intracranial pressure ( ICP ) had been increased .
	manualset3
115634	12	403579	13	NULL	NULL	0	NULL	58	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathological assessment showed that 71 ( 84 % ) victims had sustained cerebral contusions , 49 ( 58 % ) had diffuse axonal injury ( DAI ) , 57 ( 67 % ) , had ischemic brain damage ( IBD ) , 58 ( 68 % ) had symmetrical ventricular enlargement , and in 47 ( 55 % ) intracranial pressure ( ICP ) had been increased .
	manualset3
115635	13	403579	13	NULL	NULL	0	NULL	68 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathological assessment showed that 71 ( 84 % ) victims had sustained cerebral contusions , 49 ( 58 % ) had diffuse axonal injury ( DAI ) , 57 ( 67 % ) , had ischemic brain damage ( IBD ) , 58 ( 68 % ) had symmetrical ventricular enlargement , and in 47 ( 55 % ) intracranial pressure ( ICP ) had been increased .
	manualset3
115636	14	403579	13	NULL	NULL	0	NULL	symmetrical ventricular enlargement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathological assessment showed that 71 ( 84 % ) victims had sustained cerebral contusions , 49 ( 58 % ) had diffuse axonal injury ( DAI ) , 57 ( 67 % ) , had ischemic brain damage ( IBD ) , 58 ( 68 % ) had symmetrical ventricular enlargement , and in 47 ( 55 % ) intracranial pressure ( ICP ) had been increased .
	manualset3
115637	15	403579	13	NULL	NULL	0	NULL	47 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathological assessment showed that 71 ( 84 % ) victims had sustained cerebral contusions , 49 ( 58 % ) had diffuse axonal injury ( DAI ) , 57 ( 67 % ) , had ischemic brain damage ( IBD ) , 58 ( 68 % ) had symmetrical ventricular enlargement , and in 47 ( 55 % ) intracranial pressure ( ICP ) had been increased .
	manualset3
115639	16	403579	13	NULL	NULL	0	NULL	55 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathological assessment showed that 71 ( 84 % ) victims had sustained cerebral contusions , 49 ( 58 % ) had diffuse axonal injury ( DAI ) , 57 ( 67 % ) , had ischemic brain damage ( IBD ) , 58 ( 68 % ) had symmetrical ventricular enlargement , and in 47 ( 55 % ) intracranial pressure ( ICP ) had been increased .
	manualset3
115641	17	403579	13	NULL	NULL	0	NULL	intracranial pressure ( ICP )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuropathological assessment showed that 71 ( 84 % ) victims had sustained cerebral contusions , 49 ( 58 % ) had diffuse axonal injury ( DAI ) , 57 ( 67 % ) , had ischemic brain damage ( IBD ) , 58 ( 68 % ) had symmetrical ventricular enlargement , and in 47 ( 55 % ) intracranial pressure ( ICP ) had been increased .
	manualset3
115644	1	403580	13	NULL	NULL	0	NULL	Neurophysiologic and quantitative sensory testing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurophysiologic and quantitative sensory testing in the diagnosis of trigeminal neuropathy and neuropathic pain .
	manualset3
115645	2	403580	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurophysiologic and quantitative sensory testing in the diagnosis of trigeminal neuropathy and neuropathic pain .
	manualset3
115646	3	403580	13	NULL	NULL	0	NULL	trigeminal neuropathy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurophysiologic and quantitative sensory testing in the diagnosis of trigeminal neuropathy and neuropathic pain .
	manualset3
115647	4	403580	13	NULL	NULL	0	NULL	neuropathic pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurophysiologic and quantitative sensory testing in the diagnosis of trigeminal neuropathy and neuropathic pain .
	manualset3
115648	1	403581	13	NULL	NULL	0	NULL	Neuroprotective effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroprotective effect of sesame seed oil in 6-hydroxydopamine induced neurotoxicity in mice model : cellular , biochemical and neurochemical evidence .
	manualset3
115649	2	403581	13	NULL	NULL	0	NULL	sesame seed oil	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroprotective effect of sesame seed oil in 6-hydroxydopamine induced neurotoxicity in mice model : cellular , biochemical and neurochemical evidence .
	manualset3
115650	3	403581	13	NULL	NULL	0	NULL	6-hydroxydopamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroprotective effect of sesame seed oil in 6-hydroxydopamine induced neurotoxicity in mice model : cellular , biochemical and neurochemical evidence .
	manualset3
115651	4	403581	13	NULL	NULL	0	NULL	neurotoxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroprotective effect of sesame seed oil in 6-hydroxydopamine induced neurotoxicity in mice model : cellular , biochemical and neurochemical evidence .
	manualset3
115652	5	403581	13	NULL	NULL	0	NULL	mice model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroprotective effect of sesame seed oil in 6-hydroxydopamine induced neurotoxicity in mice model : cellular , biochemical and neurochemical evidence .
	manualset3
115653	6	403581	13	NULL	NULL	0	NULL	cellular evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroprotective effect of sesame seed oil in 6-hydroxydopamine induced neurotoxicity in mice model : cellular , biochemical and neurochemical evidence .
	manualset3
115654	7	403581	13	NULL	NULL	0	NULL	biochemical evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroprotective effect of sesame seed oil in 6-hydroxydopamine induced neurotoxicity in mice model : cellular , biochemical and neurochemical evidence .
	manualset3
115655	8	403581	13	NULL	NULL	0	NULL	neurochemical evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroprotective effect of sesame seed oil in 6-hydroxydopamine induced neurotoxicity in mice model : cellular , biochemical and neurochemical evidence .
	manualset3
115656	1	403582	13	NULL	NULL	0	NULL	Neurosecretory cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurosecretory cells without neurosecretion : evidence of an independently regulated trait of the cell phenotype .
	manualset3
115657	2	403582	13	NULL	NULL	0	NULL	neurosecretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurosecretory cells without neurosecretion : evidence of an independently regulated trait of the cell phenotype .
	manualset3
115658	3	403582	13	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurosecretory cells without neurosecretion : evidence of an independently regulated trait of the cell phenotype .
	manualset3
115659	4	403582	13	NULL	NULL	0	NULL	trait 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurosecretory cells without neurosecretion : evidence of an independently regulated trait of the cell phenotype .
	manualset3
115660	5	403582	13	NULL	NULL	0	NULL	cell phenotype	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurosecretory cells without neurosecretion : evidence of an independently regulated trait of the cell phenotype .
	manualset3
115661	1	403583	13	NULL	NULL	0	NULL	Neurosurgical watch sheet 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurosurgical watch sheet for craniocerebral trauma .
	manualset3
115662	2	403583	13	NULL	NULL	0	NULL	craniocerebral trauma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurosurgical watch sheet for craniocerebral trauma .
	manualset3
115663	1	403584	13	NULL	NULL	0	NULL	Neurotherapeutics 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurotherapeutics to inhibit exocytosis from sensory neurons for the control of chronic pain .
	manualset3
115664	2	403584	13	NULL	NULL	0	NULL	exocytosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurotherapeutics to inhibit exocytosis from sensory neurons for the control of chronic pain .
	manualset3
115665	3	403584	13	NULL	NULL	0	NULL	sensory neurons 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurotherapeutics to inhibit exocytosis from sensory neurons for the control of chronic pain .
	manualset3
115666	4	403584	13	NULL	NULL	0	NULL	control 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurotherapeutics to inhibit exocytosis from sensory neurons for the control of chronic pain .
	manualset3
115667	5	403584	13	NULL	NULL	0	NULL	chronic pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurotherapeutics to inhibit exocytosis from sensory neurons for the control of chronic pain .
	manualset3
115668	1	403585	13	NULL	NULL	0	NULL	Neutral , volatile polyfluorinated alkyl substances ( PFAS )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutral , volatile polyfluorinated alkyl substances ( PFAS ) were determined in high-volume air samples collected onboard the German research vessel Polarstern during cruise ANTXXIII-1 between Bremerhaven , Germany ( 53 degrees N ) and Capetown , Republic of South Africa ( 33 degrees S ) in fall 2005 .
	manualset3
115669	2	403585	13	NULL	NULL	0	NULL	high-volume air samples 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutral , volatile polyfluorinated alkyl substances ( PFAS ) were determined in high-volume air samples collected onboard the German research vessel Polarstern during cruise ANTXXIII-1 between Bremerhaven , Germany ( 53 degrees N ) and Capetown , Republic of South Africa ( 33 degrees S ) in fall 2005 .
	manualset3
115670	3	403585	13	NULL	NULL	0	NULL	 German research vessel Polarstern	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutral , volatile polyfluorinated alkyl substances ( PFAS ) were determined in high-volume air samples collected onboard the German research vessel Polarstern during cruise ANTXXIII-1 between Bremerhaven , Germany ( 53 degrees N ) and Capetown , Republic of South Africa ( 33 degrees S ) in fall 2005 .
	manualset3
115671	4	403585	13	NULL	NULL	0	NULL	cruise ANTXXIII-1 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutral , volatile polyfluorinated alkyl substances ( PFAS ) were determined in high-volume air samples collected onboard the German research vessel Polarstern during cruise ANTXXIII-1 between Bremerhaven , Germany ( 53 degrees N ) and Capetown , Republic of South Africa ( 33 degrees S ) in fall 2005 .
	manualset3
115672	5	403585	13	NULL	NULL	0	NULL	Bremerhaven	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutral , volatile polyfluorinated alkyl substances ( PFAS ) were determined in high-volume air samples collected onboard the German research vessel Polarstern during cruise ANTXXIII-1 between Bremerhaven , Germany ( 53 degrees N ) and Capetown , Republic of South Africa ( 33 degrees S ) in fall 2005 .
	manualset3
115673	6	403585	13	NULL	NULL	0	NULL	Germany	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutral , volatile polyfluorinated alkyl substances ( PFAS ) were determined in high-volume air samples collected onboard the German research vessel Polarstern during cruise ANTXXIII-1 between Bremerhaven , Germany ( 53 degrees N ) and Capetown , Republic of South Africa ( 33 degrees S ) in fall 2005 .
	manualset3
115674	7	403585	13	NULL	NULL	0	NULL	53 degrees N	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutral , volatile polyfluorinated alkyl substances ( PFAS ) were determined in high-volume air samples collected onboard the German research vessel Polarstern during cruise ANTXXIII-1 between Bremerhaven , Germany ( 53 degrees N ) and Capetown , Republic of South Africa ( 33 degrees S ) in fall 2005 .
	manualset3
115675	8	403585	13	NULL	NULL	0	NULL	Capetown	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutral , volatile polyfluorinated alkyl substances ( PFAS ) were determined in high-volume air samples collected onboard the German research vessel Polarstern during cruise ANTXXIII-1 between Bremerhaven , Germany ( 53 degrees N ) and Capetown , Republic of South Africa ( 33 degrees S ) in fall 2005 .
	manualset3
115676	9	403585	13	NULL	NULL	0	NULL	Republic of South Africa 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutral , volatile polyfluorinated alkyl substances ( PFAS ) were determined in high-volume air samples collected onboard the German research vessel Polarstern during cruise ANTXXIII-1 between Bremerhaven , Germany ( 53 degrees N ) and Capetown , Republic of South Africa ( 33 degrees S ) in fall 2005 .
	manualset3
115677	10	403585	13	NULL	NULL	0	NULL	33 degrees S 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutral , volatile polyfluorinated alkyl substances ( PFAS ) were determined in high-volume air samples collected onboard the German research vessel Polarstern during cruise ANTXXIII-1 between Bremerhaven , Germany ( 53 degrees N ) and Capetown , Republic of South Africa ( 33 degrees S ) in fall 2005 .
	manualset3
115678	11	403585	13	NULL	NULL	0	NULL	fall 2005 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutral , volatile polyfluorinated alkyl substances ( PFAS ) were determined in high-volume air samples collected onboard the German research vessel Polarstern during cruise ANTXXIII-1 between Bremerhaven , Germany ( 53 degrees N ) and Capetown , Republic of South Africa ( 33 degrees S ) in fall 2005 .
	manualset3
115679	1	403586	13	NULL	NULL	0	NULL	Neutralisation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutralisation of the pathological effects of venoms from E. ocellatus , B. arietans and N. nigricollis by IgG from the venom-immunised camels , or commercial antivenom , was compared using assays of venom lethality ( ED ( 50 ) ) , hemorrhage ( MHD ) and coagulopathy ( MCD ) .
	manualset3
115680	2	403586	13	NULL	NULL	0	NULL	pathological effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutralisation of the pathological effects of venoms from E. ocellatus , B. arietans and N. nigricollis by IgG from the venom-immunised camels , or commercial antivenom , was compared using assays of venom lethality ( ED ( 50 ) ) , hemorrhage ( MHD ) and coagulopathy ( MCD ) .
	manualset3
115681	3	403586	13	NULL	NULL	0	NULL	venoms 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutralisation of the pathological effects of venoms from E. ocellatus , B. arietans and N. nigricollis by IgG from the venom-immunised camels , or commercial antivenom , was compared using assays of venom lethality ( ED ( 50 ) ) , hemorrhage ( MHD ) and coagulopathy ( MCD ) .
	manualset3
115682	4	403586	13	NULL	NULL	0	NULL	E. ocellatus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutralisation of the pathological effects of venoms from E. ocellatus , B. arietans and N. nigricollis by IgG from the venom-immunised camels , or commercial antivenom , was compared using assays of venom lethality ( ED ( 50 ) ) , hemorrhage ( MHD ) and coagulopathy ( MCD ) .
	manualset3
115683	5	403586	13	NULL	NULL	0	NULL	B. arietans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutralisation of the pathological effects of venoms from E. ocellatus , B. arietans and N. nigricollis by IgG from the venom-immunised camels , or commercial antivenom , was compared using assays of venom lethality ( ED ( 50 ) ) , hemorrhage ( MHD ) and coagulopathy ( MCD ) .
	manualset3
115684	6	403586	13	NULL	NULL	0	NULL	N. nigricollis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutralisation of the pathological effects of venoms from E. ocellatus , B. arietans and N. nigricollis by IgG from the venom-immunised camels , or commercial antivenom , was compared using assays of venom lethality ( ED ( 50 ) ) , hemorrhage ( MHD ) and coagulopathy ( MCD ) .
	manualset3
115685	7	403586	13	NULL	NULL	0	NULL	IgG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutralisation of the pathological effects of venoms from E. ocellatus , B. arietans and N. nigricollis by IgG from the venom-immunised camels , or commercial antivenom , was compared using assays of venom lethality ( ED ( 50 ) ) , hemorrhage ( MHD ) and coagulopathy ( MCD ) .
	manualset3
115686	8	403586	13	NULL	NULL	0	NULL	venom-immunised camels	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutralisation of the pathological effects of venoms from E. ocellatus , B. arietans and N. nigricollis by IgG from the venom-immunised camels , or commercial antivenom , was compared using assays of venom lethality ( ED ( 50 ) ) , hemorrhage ( MHD ) and coagulopathy ( MCD ) .
	manualset3
115687	9	403586	13	NULL	NULL	0	NULL	commercial antivenom	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutralisation of the pathological effects of venoms from E. ocellatus , B. arietans and N. nigricollis by IgG from the venom-immunised camels , or commercial antivenom , was compared using assays of venom lethality ( ED ( 50 ) ) , hemorrhage ( MHD ) and coagulopathy ( MCD ) .
	manualset3
115688	10	403586	13	NULL	NULL	0	NULL	assays of venom lethality	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutralisation of the pathological effects of venoms from E. ocellatus , B. arietans and N. nigricollis by IgG from the venom-immunised camels , or commercial antivenom , was compared using assays of venom lethality ( ED ( 50 ) ) , hemorrhage ( MHD ) and coagulopathy ( MCD ) .
	manualset3
115689	11	403586	13	NULL	NULL	0	NULL	ED ( 50 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutralisation of the pathological effects of venoms from E. ocellatus , B. arietans and N. nigricollis by IgG from the venom-immunised camels , or commercial antivenom , was compared using assays of venom lethality ( ED ( 50 ) ) , hemorrhage ( MHD ) and coagulopathy ( MCD ) .
	manualset3
115690	12	403586	13	NULL	NULL	0	NULL	hemorrhage ( MHD )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutralisation of the pathological effects of venoms from E. ocellatus , B. arietans and N. nigricollis by IgG from the venom-immunised camels , or commercial antivenom , was compared using assays of venom lethality ( ED ( 50 ) ) , hemorrhage ( MHD ) and coagulopathy ( MCD ) .
	manualset3
115691	13	403586	13	NULL	NULL	0	NULL	coagulopathy ( MCD )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutralisation of the pathological effects of venoms from E. ocellatus , B. arietans and N. nigricollis by IgG from the venom-immunised camels , or commercial antivenom , was compared using assays of venom lethality ( ED ( 50 ) ) , hemorrhage ( MHD ) and coagulopathy ( MCD ) .
	manualset3
115692	1	403587	13	NULL	NULL	0	NULL	Neutralizing activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutralizing activity of sera from guinea-pigs inoculated with foot-and-mouth disease virus variants .
	manualset3
115693	2	403587	13	NULL	NULL	0	NULL	sera	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutralizing activity of sera from guinea-pigs inoculated with foot-and-mouth disease virus variants .
	manualset3
115694	3	403587	13	NULL	NULL	0	NULL	guinea-pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutralizing activity of sera from guinea-pigs inoculated with foot-and-mouth disease virus variants .
	manualset3
115695	4	403587	13	NULL	NULL	0	NULL	foot-and-mouth disease virus variants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutralizing activity of sera from guinea-pigs inoculated with foot-and-mouth disease virus variants .
	manualset3
115696	1	403588	13	NULL	NULL	0	NULL	anatomy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( 2 ) Since anatomy is sectionalized , understanding of the body is dwarfed and distorted .
	manualset3
115697	2	403588	13	NULL	NULL	0	NULL	understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( 2 ) Since anatomy is sectionalized , understanding of the body is dwarfed and distorted .
	manualset3
115698	3	403588	13	NULL	NULL	0	NULL	body	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( 2 ) Since anatomy is sectionalized , understanding of the body is dwarfed and distorted .
	manualset3
115699	1	403589	13	NULL	NULL	0	NULL	comparison 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of models with only cytology variables versus models with both cytology and QFIA variables indicated that the QFIA provided an important additional predictive value .
	manualset3
115700	2	403589	13	NULL	NULL	0	NULL	models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of models with only cytology variables versus models with both cytology and QFIA variables indicated that the QFIA provided an important additional predictive value .
	manualset3
115701	3	403589	13	NULL	NULL	0	NULL	cytology variables 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of models with only cytology variables versus models with both cytology and QFIA variables indicated that the QFIA provided an important additional predictive value .
	manualset3
115702	4	403589	13	NULL	NULL	0	NULL	models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of models with only cytology variables versus models with both cytology and QFIA variables indicated that the QFIA provided an important additional predictive value .
	manualset3
115703	5	403589	13	NULL	NULL	0	NULL	cytology variables	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of models with only cytology variables versus models with both cytology and QFIA variables indicated that the QFIA provided an important additional predictive value .
	manualset3
115704	6	403589	13	NULL	NULL	0	NULL	QFIA variables	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of models with only cytology variables versus models with both cytology and QFIA variables indicated that the QFIA provided an important additional predictive value .
	manualset3
115705	7	403589	13	NULL	NULL	0	NULL	QFIA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of models with only cytology variables versus models with both cytology and QFIA variables indicated that the QFIA provided an important additional predictive value .
	manualset3
115706	8	403589	13	NULL	NULL	0	NULL	predictive value	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of models with only cytology variables versus models with both cytology and QFIA variables indicated that the QFIA provided an important additional predictive value .
	manualset3
115707	1	403590	13	NULL	NULL	0	NULL	Neutrophil-derived oxygen metabolites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutrophil-derived oxygen metabolites are thought to play an important role in the genesis of acute lung injury in a variety of diseases .
	manualset3
115708	2	403590	13	NULL	NULL	0	NULL	important role 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutrophil-derived oxygen metabolites are thought to play an important role in the genesis of acute lung injury in a variety of diseases .
	manualset3
115709	3	403590	13	NULL	NULL	0	NULL	genesis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutrophil-derived oxygen metabolites are thought to play an important role in the genesis of acute lung injury in a variety of diseases .
	manualset3
115710	4	403590	13	NULL	NULL	0	NULL	acute lung injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutrophil-derived oxygen metabolites are thought to play an important role in the genesis of acute lung injury in a variety of diseases .
	manualset3
115711	5	403590	13	NULL	NULL	0	NULL	diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutrophil-derived oxygen metabolites are thought to play an important role in the genesis of acute lung injury in a variety of diseases .
	manualset3
115712	1	403591	13	NULL	NULL	0	NULL	Neutrophil	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutrophil depletion with mechlorethamine ( 0.75 mg/kg iv ) significantly reduced the extent of necrosis in pig LD muscles .
	manualset3
115713	2	403591	13	NULL	NULL	0	NULL	depletion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutrophil depletion with mechlorethamine ( 0.75 mg/kg iv ) significantly reduced the extent of necrosis in pig LD muscles .
	manualset3
115714	3	403591	13	NULL	NULL	0	NULL	mechlorethamine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutrophil depletion with mechlorethamine ( 0.75 mg/kg iv ) significantly reduced the extent of necrosis in pig LD muscles .
	manualset3
115715	4	403591	13	NULL	NULL	0	NULL	0.75 mg/kg iv 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutrophil depletion with mechlorethamine ( 0.75 mg/kg iv ) significantly reduced the extent of necrosis in pig LD muscles .
	manualset3
115716	5	403591	13	NULL	NULL	0	NULL	extent of necrosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutrophil depletion with mechlorethamine ( 0.75 mg/kg iv ) significantly reduced the extent of necrosis in pig LD muscles .
	manualset3
115717	6	403591	13	NULL	NULL	0	NULL	pig LD muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutrophil depletion with mechlorethamine ( 0.75 mg/kg iv ) significantly reduced the extent of necrosis in pig LD muscles .
	manualset3
115718	1	403592	13	NULL	NULL	0	NULL	Neutrophil 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutrophil recruitment and bacterial clearance correlated with LPS responsiveness in local gram-negative infection .
	manualset3
115719	2	403592	13	NULL	NULL	0	NULL	recruitment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutrophil recruitment and bacterial clearance correlated with LPS responsiveness in local gram-negative infection .
	manualset3
115720	3	403592	13	NULL	NULL	0	NULL	bacterial clearance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutrophil recruitment and bacterial clearance correlated with LPS responsiveness in local gram-negative infection .
	manualset3
115721	4	403592	13	NULL	NULL	0	NULL	LPS responsiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutrophil recruitment and bacterial clearance correlated with LPS responsiveness in local gram-negative infection .
	manualset3
115722	5	403592	13	NULL	NULL	0	NULL	local gram-negative infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neutrophil recruitment and bacterial clearance correlated with LPS responsiveness in local gram-negative infection .
	manualset3
115723	1	403593	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Never before have patients had access to so much information ( and misinformation ) about treatment , options , materials , and alternatives .
	manualset3
115724	2	403593	13	NULL	NULL	0	NULL	access 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Never before have patients had access to so much information ( and misinformation ) about treatment , options , materials , and alternatives .
	manualset3
115725	3	403593	13	NULL	NULL	0	NULL	information 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Never before have patients had access to so much information ( and misinformation ) about treatment , options , materials , and alternatives .
	manualset3
115726	4	403593	13	NULL	NULL	0	NULL	misinformation	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Never before have patients had access to so much information ( and misinformation ) about treatment , options , materials , and alternatives .
	manualset3
115727	5	403593	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Never before have patients had access to so much information ( and misinformation ) about treatment , options , materials , and alternatives .
	manualset3
115728	6	403593	13	NULL	NULL	0	NULL	options	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Never before have patients had access to so much information ( and misinformation ) about treatment , options , materials , and alternatives .
	manualset3
115729	7	403593	13	NULL	NULL	0	NULL	materials	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Never before have patients had access to so much information ( and misinformation ) about treatment , options , materials , and alternatives .
	manualset3
115730	8	403593	13	NULL	NULL	0	NULL	alternatives 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Never before have patients had access to so much information ( and misinformation ) about treatment , options , materials , and alternatives .
	manualset3
115731	1	403594	13	NULL	NULL	0	NULL	immunization 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , a single immunization with both mutant strains ( EGDe DeltaactA2 and DeltaactADeltaplcB ) efficiently induced and maintained effector memory ( CD8 ( + ) ) T cells and has provided animals with a state of long-lasting protective immunity against wild type L. monocytogenes .
	manualset3
115732	2	403594	13	NULL	NULL	0	NULL	mutant strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , a single immunization with both mutant strains ( EGDe DeltaactA2 and DeltaactADeltaplcB ) efficiently induced and maintained effector memory ( CD8 ( + ) ) T cells and has provided animals with a state of long-lasting protective immunity against wild type L. monocytogenes .
	manualset3
115733	3	403594	13	NULL	NULL	0	NULL	EGDe DeltaactA2	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , a single immunization with both mutant strains ( EGDe DeltaactA2 and DeltaactADeltaplcB ) efficiently induced and maintained effector memory ( CD8 ( + ) ) T cells and has provided animals with a state of long-lasting protective immunity against wild type L. monocytogenes .
	manualset3
115734	4	403594	13	NULL	NULL	0	NULL	DeltaactADeltaplcB 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , a single immunization with both mutant strains ( EGDe DeltaactA2 and DeltaactADeltaplcB ) efficiently induced and maintained effector memory ( CD8 ( + ) ) T cells and has provided animals with a state of long-lasting protective immunity against wild type L. monocytogenes .
	manualset3
115735	5	403594	13	NULL	NULL	0	NULL	effector memory	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , a single immunization with both mutant strains ( EGDe DeltaactA2 and DeltaactADeltaplcB ) efficiently induced and maintained effector memory ( CD8 ( + ) ) T cells and has provided animals with a state of long-lasting protective immunity against wild type L. monocytogenes .
	manualset3
115736	6	403594	13	NULL	NULL	0	NULL	CD8 ( + ) ) T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , a single immunization with both mutant strains ( EGDe DeltaactA2 and DeltaactADeltaplcB ) efficiently induced and maintained effector memory ( CD8 ( + ) ) T cells and has provided animals with a state of long-lasting protective immunity against wild type L. monocytogenes .
	manualset3
115737	7	403594	13	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , a single immunization with both mutant strains ( EGDe DeltaactA2 and DeltaactADeltaplcB ) efficiently induced and maintained effector memory ( CD8 ( + ) ) T cells and has provided animals with a state of long-lasting protective immunity against wild type L. monocytogenes .
	manualset3
115738	8	403594	13	NULL	NULL	0	NULL	protective immunity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , a single immunization with both mutant strains ( EGDe DeltaactA2 and DeltaactADeltaplcB ) efficiently induced and maintained effector memory ( CD8 ( + ) ) T cells and has provided animals with a state of long-lasting protective immunity against wild type L. monocytogenes .
	manualset3
115739	9	403594	13	NULL	NULL	0	NULL	wild type L. monocytogenes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , a single immunization with both mutant strains ( EGDe DeltaactA2 and DeltaactADeltaplcB ) efficiently induced and maintained effector memory ( CD8 ( + ) ) T cells and has provided animals with a state of long-lasting protective immunity against wild type L. monocytogenes .
	manualset3
119330	10	403594	13	NULL	NULL	0	NULL	state	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , a single immunization with both mutant strains ( EGDe DeltaactA2 and DeltaactADeltaplcB ) efficiently induced and maintained effector memory ( CD8 ( + ) ) T cells and has provided animals with a state of long-lasting protective immunity against wild type L. monocytogenes .
	manualset3
115740	1	403595	13	NULL	NULL	NULL	NULL	age-related differences	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nevertheless , age-related differences in the relative activation of components of emotion processing networks are poorly understood .
	manualset3
115741	2	403595	13	NULL	NULL	0	NULL	relative activation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , age-related differences in the relative activation of components of emotion processing networks are poorly understood .
	manualset3
115742	3	403595	13	NULL	NULL	0	NULL	components	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , age-related differences in the relative activation of components of emotion processing networks are poorly understood .
	manualset3
115743	4	403595	13	NULL	NULL	0	NULL	emotion processing networks 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , age-related differences in the relative activation of components of emotion processing networks are poorly understood .
	manualset3
115744	1	403596	13	NULL	NULL	0	NULL	astrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , astrocytes retain the expression of non-homologous end-joining ( NHEJ ) genes and indeed they are DNA repair proficient .
	manualset3
115745	2	403596	13	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , astrocytes retain the expression of non-homologous end-joining ( NHEJ ) genes and indeed they are DNA repair proficient .
	manualset3
115746	3	403596	13	NULL	NULL	0	NULL	 non-homologous end-joining ( NHEJ ) genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , astrocytes retain the expression of non-homologous end-joining ( NHEJ ) genes and indeed they are DNA repair proficient .
	manualset3
115747	4	403596	13	NULL	NULL	0	NULL	DNA repair	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , astrocytes retain the expression of non-homologous end-joining ( NHEJ ) genes and indeed they are DNA repair proficient .
	manualset3
115748	1	403597	13	NULL	NULL	0	NULL	clinicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , clinicians must keep in mind the simplicity and the effectiveness of iodine prophylaxis .
	manualset3
115749	2	403597	13	NULL	NULL	0	NULL	mind	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , clinicians must keep in mind the simplicity and the effectiveness of iodine prophylaxis .
	manualset3
115750	3	403597	13	NULL	NULL	0	NULL	simplicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , clinicians must keep in mind the simplicity and the effectiveness of iodine prophylaxis .
	manualset3
115751	4	403597	13	NULL	NULL	0	NULL	effectiveness 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , clinicians must keep in mind the simplicity and the effectiveness of iodine prophylaxis .
	manualset3
115752	5	403597	13	NULL	NULL	0	NULL	iodine prophylaxis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , clinicians must keep in mind the simplicity and the effectiveness of iodine prophylaxis .
	manualset3
115753	1	403598	13	NULL	NULL	0	NULL	countries	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , countries were able to capitalize on the infrastructure of their immunization programs and widespread experience utilizing the seasonal influenza vaccine to prepare rapidly , developing H1N1 vaccination plans targeting individuals with chronic disease , pregnant women and health care workers , among others .
	manualset3
115754	2	403598	13	NULL	NULL	0	NULL	infrastructure	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , countries were able to capitalize on the infrastructure of their immunization programs and widespread experience utilizing the seasonal influenza vaccine to prepare rapidly , developing H1N1 vaccination plans targeting individuals with chronic disease , pregnant women and health care workers , among others .
	manualset3
115755	3	403598	13	NULL	NULL	0	NULL	immunization programs 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , countries were able to capitalize on the infrastructure of their immunization programs and widespread experience utilizing the seasonal influenza vaccine to prepare rapidly , developing H1N1 vaccination plans targeting individuals with chronic disease , pregnant women and health care workers , among others .
	manualset3
115756	4	403598	13	NULL	NULL	0	NULL	widespread experience	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , countries were able to capitalize on the infrastructure of their immunization programs and widespread experience utilizing the seasonal influenza vaccine to prepare rapidly , developing H1N1 vaccination plans targeting individuals with chronic disease , pregnant women and health care workers , among others .
	manualset3
115757	5	403598	13	NULL	NULL	0	NULL	 seasonal influenza vaccine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , countries were able to capitalize on the infrastructure of their immunization programs and widespread experience utilizing the seasonal influenza vaccine to prepare rapidly , developing H1N1 vaccination plans targeting individuals with chronic disease , pregnant women and health care workers , among others .
	manualset3
115758	6	403598	13	NULL	NULL	0	NULL	H1N1 vaccination plans	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , countries were able to capitalize on the infrastructure of their immunization programs and widespread experience utilizing the seasonal influenza vaccine to prepare rapidly , developing H1N1 vaccination plans targeting individuals with chronic disease , pregnant women and health care workers , among others .
	manualset3
115759	7	403598	13	NULL	NULL	0	NULL	individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , countries were able to capitalize on the infrastructure of their immunization programs and widespread experience utilizing the seasonal influenza vaccine to prepare rapidly , developing H1N1 vaccination plans targeting individuals with chronic disease , pregnant women and health care workers , among others .
	manualset3
115760	8	403598	13	NULL	NULL	0	NULL	chronic disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , countries were able to capitalize on the infrastructure of their immunization programs and widespread experience utilizing the seasonal influenza vaccine to prepare rapidly , developing H1N1 vaccination plans targeting individuals with chronic disease , pregnant women and health care workers , among others .
	manualset3
115761	9	403598	13	NULL	NULL	0	NULL	pregnant women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , countries were able to capitalize on the infrastructure of their immunization programs and widespread experience utilizing the seasonal influenza vaccine to prepare rapidly , developing H1N1 vaccination plans targeting individuals with chronic disease , pregnant women and health care workers , among others .
	manualset3
115762	10	403598	13	NULL	NULL	0	NULL	health care workers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , countries were able to capitalize on the infrastructure of their immunization programs and widespread experience utilizing the seasonal influenza vaccine to prepare rapidly , developing H1N1 vaccination plans targeting individuals with chronic disease , pregnant women and health care workers , among others .
	manualset3
115763	11	403598	13	NULL	NULL	0	NULL	others	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , countries were able to capitalize on the infrastructure of their immunization programs and widespread experience utilizing the seasonal influenza vaccine to prepare rapidly , developing H1N1 vaccination plans targeting individuals with chronic disease , pregnant women and health care workers , among others .
	manualset3
115764	1	403599	13	NULL	NULL	0	NULL	enucleation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , enucleation of the affected eye often is inevitable .
	manualset3
115765	2	403599	13	NULL	NULL	0	NULL	eye	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , enucleation of the affected eye often is inevitable .
	manualset3
115766	1	403600	13	NULL	NULL	0	NULL	few articles	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , few articles are available that combine the interdisciplinary fields of medicine , genetics , physiology , and statistics in order to provide the scientific rationale for such an endeavor .
	manualset3
115767	2	403600	13	NULL	NULL	0	NULL	interdisciplinary fields 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , few articles are available that combine the interdisciplinary fields of medicine , genetics , physiology , and statistics in order to provide the scientific rationale for such an endeavor .
	manualset3
115768	3	403600	13	NULL	NULL	0	NULL	medicine	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , few articles are available that combine the interdisciplinary fields of medicine , genetics , physiology , and statistics in order to provide the scientific rationale for such an endeavor .
	manualset3
115769	4	403600	13	NULL	NULL	0	NULL	genetics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , few articles are available that combine the interdisciplinary fields of medicine , genetics , physiology , and statistics in order to provide the scientific rationale for such an endeavor .
	manualset3
115770	5	403600	13	NULL	NULL	0	NULL	physiology 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , few articles are available that combine the interdisciplinary fields of medicine , genetics , physiology , and statistics in order to provide the scientific rationale for such an endeavor .
	manualset3
115771	6	403600	13	NULL	NULL	0	NULL	statistics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , few articles are available that combine the interdisciplinary fields of medicine , genetics , physiology , and statistics in order to provide the scientific rationale for such an endeavor .
	manualset3
115772	7	403600	13	NULL	NULL	0	NULL	scientific rationale	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , few articles are available that combine the interdisciplinary fields of medicine , genetics , physiology , and statistics in order to provide the scientific rationale for such an endeavor .
	manualset3
115773	8	403600	13	NULL	NULL	0	NULL	endeavor	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , few articles are available that combine the interdisciplinary fields of medicine , genetics , physiology , and statistics in order to provide the scientific rationale for such an endeavor .
	manualset3
115831	1	403601	13	NULL	NULL	0	NULL	PCR products 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , longer PCR products can be sequenced by serial bisulphite pyrosequencing , which utilises tandem assays along the amplicon .
	manualset3
115832	2	403601	13	NULL	NULL	0	NULL	serial bisulphite pyrosequencing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , longer PCR products can be sequenced by serial bisulphite pyrosequencing , which utilises tandem assays along the amplicon .
	manualset3
115833	3	403601	13	NULL	NULL	0	NULL	tandem assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , longer PCR products can be sequenced by serial bisulphite pyrosequencing , which utilises tandem assays along the amplicon .
	manualset3
115834	4	403601	13	NULL	NULL	0	NULL	amplicon	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , longer PCR products can be sequenced by serial bisulphite pyrosequencing , which utilises tandem assays along the amplicon .
	manualset3
115835	1	403602	13	NULL	NULL	0	NULL	emphasis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , major emphasis is placed on the group of Annexin V-based radioligands , in particular ( 99m ) Tc-Hynic-Annexin V , since this molecule is by far the most extensively investigated and best-characterised apoptosis marker at present .
	manualset3
115836	2	403602	13	NULL	NULL	0	NULL	 group of Annexin V-based radioligands	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , major emphasis is placed on the group of Annexin V-based radioligands , in particular ( 99m ) Tc-Hynic-Annexin V , since this molecule is by far the most extensively investigated and best-characterised apoptosis marker at present .
	manualset3
115837	3	403602	13	NULL	NULL	0	NULL	( 99m ) Tc-Hynic-Annexin V	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , major emphasis is placed on the group of Annexin V-based radioligands , in particular ( 99m ) Tc-Hynic-Annexin V , since this molecule is by far the most extensively investigated and best-characterised apoptosis marker at present .
	manualset3
115838	4	403602	13	NULL	NULL	0	NULL	molecule	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , major emphasis is placed on the group of Annexin V-based radioligands , in particular ( 99m ) Tc-Hynic-Annexin V , since this molecule is by far the most extensively investigated and best-characterised apoptosis marker at present .
	manualset3
115839	5	403602	13	NULL	NULL	0	NULL	apoptosis marker	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , major emphasis is placed on the group of Annexin V-based radioligands , in particular ( 99m ) Tc-Hynic-Annexin V , since this molecule is by far the most extensively investigated and best-characterised apoptosis marker at present .
	manualset3
115840	1	403603	13	NULL	NULL	0	NULL	concerns	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , one of the main concerns remains the potential interference between both modalities leading to an increased toxicity , which may outweigh all potential benefit .
	manualset3
115841	2	403603	13	NULL	NULL	0	NULL	potential interference 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , one of the main concerns remains the potential interference between both modalities leading to an increased toxicity , which may outweigh all potential benefit .
	manualset3
115842	3	403603	13	NULL	NULL	0	NULL	toxicity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , one of the main concerns remains the potential interference between both modalities leading to an increased toxicity , which may outweigh all potential benefit .
	manualset3
115843	4	403603	13	NULL	NULL	0	NULL	potential benefit 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , one of the main concerns remains the potential interference between both modalities leading to an increased toxicity , which may outweigh all potential benefit .
	manualset3
115844	5	403603	13	NULL	NULL	0	NULL	modalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , one of the main concerns remains the potential interference between both modalities leading to an increased toxicity , which may outweigh all potential benefit .
	manualset3
115853	1	403604	13	NULL	NULL	0	NULL	telomere	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , progressive telomere shortening in the mutants , however slow , ultimately should be lethal .
	manualset3
115860	2	403604	13	NULL	NULL	0	NULL	mutants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , progressive telomere shortening in the mutants , however slow , ultimately should be lethal .
	manualset3
115863	1	403605	13	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , results from this study , together with those from a number of comparable studies , indicate that peptide vaccines are currently of minimal benefit to patients and support the need for ongoing development of new strategies in treatment of this disease .
	manualset3
115864	2	403605	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , results from this study , together with those from a number of comparable studies , indicate that peptide vaccines are currently of minimal benefit to patients and support the need for ongoing development of new strategies in treatment of this disease .
	manualset3
115867	3	403605	13	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , results from this study , together with those from a number of comparable studies , indicate that peptide vaccines are currently of minimal benefit to patients and support the need for ongoing development of new strategies in treatment of this disease .
	manualset3
115868	4	403605	13	NULL	NULL	0	NULL	comparable studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , results from this study , together with those from a number of comparable studies , indicate that peptide vaccines are currently of minimal benefit to patients and support the need for ongoing development of new strategies in treatment of this disease .
	manualset3
115869	5	403605	13	NULL	NULL	0	NULL	peptide vaccines 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , results from this study , together with those from a number of comparable studies , indicate that peptide vaccines are currently of minimal benefit to patients and support the need for ongoing development of new strategies in treatment of this disease .
	manualset3
115870	6	403605	13	NULL	NULL	0	NULL	benefit	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , results from this study , together with those from a number of comparable studies , indicate that peptide vaccines are currently of minimal benefit to patients and support the need for ongoing development of new strategies in treatment of this disease .
	manualset3
115871	7	403605	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , results from this study , together with those from a number of comparable studies , indicate that peptide vaccines are currently of minimal benefit to patients and support the need for ongoing development of new strategies in treatment of this disease .
	manualset3
115872	8	403605	13	NULL	NULL	0	NULL	need	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , results from this study , together with those from a number of comparable studies , indicate that peptide vaccines are currently of minimal benefit to patients and support the need for ongoing development of new strategies in treatment of this disease .
	manualset3
115873	9	403605	13	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , results from this study , together with those from a number of comparable studies , indicate that peptide vaccines are currently of minimal benefit to patients and support the need for ongoing development of new strategies in treatment of this disease .
	manualset3
115874	10	403605	13	NULL	NULL	0	NULL	strategies	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , results from this study , together with those from a number of comparable studies , indicate that peptide vaccines are currently of minimal benefit to patients and support the need for ongoing development of new strategies in treatment of this disease .
	manualset3
115875	11	403605	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , results from this study , together with those from a number of comparable studies , indicate that peptide vaccines are currently of minimal benefit to patients and support the need for ongoing development of new strategies in treatment of this disease .
	manualset3
115876	12	403605	13	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , results from this study , together with those from a number of comparable studies , indicate that peptide vaccines are currently of minimal benefit to patients and support the need for ongoing development of new strategies in treatment of this disease .
	manualset3
115913	1	403606	13	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of the cardiovascular responses to treadmill and bicycle ergometer exercise in healthy male Nigerians .
	manualset3
115915	2	403606	13	NULL	NULL	0	NULL	 cardiovascular responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of the cardiovascular responses to treadmill and bicycle ergometer exercise in healthy male Nigerians .
	manualset3
115916	3	403606	13	NULL	NULL	0	NULL	treadmill 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of the cardiovascular responses to treadmill and bicycle ergometer exercise in healthy male Nigerians .
	manualset3
115919	4	403606	13	NULL	NULL	0	NULL	bicycle ergometer exercise	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of the cardiovascular responses to treadmill and bicycle ergometer exercise in healthy male Nigerians .
	manualset3
115922	5	403606	13	NULL	NULL	0	NULL	healthy male Nigerians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of the cardiovascular responses to treadmill and bicycle ergometer exercise in healthy male Nigerians .
	manualset3
115961	1	403607	13	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nevertheless , some patients exhibit high residual P5 ` N-1 activity , suggesting that P5 ` N-1 deficiency is compensate by other nucleotidases and/or alternative pathways in nucleotide metabolism .
	manualset3
115962	2	403607	13	NULL	NULL	0	NULL	 residual P5 ` N-1 activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , some patients exhibit high residual P5 ` N-1 activity , suggesting that P5 ` N-1 deficiency is compensate by other nucleotidases and/or alternative pathways in nucleotide metabolism .
	manualset3
115963	3	403607	13	NULL	NULL	0	NULL	P5 ` N-1 deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , some patients exhibit high residual P5 ` N-1 activity , suggesting that P5 ` N-1 deficiency is compensate by other nucleotidases and/or alternative pathways in nucleotide metabolism .
	manualset3
115964	4	403607	13	NULL	NULL	0	NULL	nucleotidases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , some patients exhibit high residual P5 ` N-1 activity , suggesting that P5 ` N-1 deficiency is compensate by other nucleotidases and/or alternative pathways in nucleotide metabolism .
	manualset3
115965	5	403607	13	NULL	NULL	0	NULL	alternative pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , some patients exhibit high residual P5 ` N-1 activity , suggesting that P5 ` N-1 deficiency is compensate by other nucleotidases and/or alternative pathways in nucleotide metabolism .
	manualset3
115966	6	403607	13	NULL	NULL	0	NULL	nucleotide metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , some patients exhibit high residual P5 ` N-1 activity , suggesting that P5 ` N-1 deficiency is compensate by other nucleotidases and/or alternative pathways in nucleotide metabolism .
	manualset3
115967	1	403608	13	NULL	NULL	0	NULL	Ad5-p53-induced apoptosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the Ad5-p53-induced apoptosis was partially inhibited when Ad5-Rb was added simultaneously .
	manualset3
115968	2	403608	13	NULL	NULL	0	NULL	Ad5-Rb 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the Ad5-p53-induced apoptosis was partially inhibited when Ad5-Rb was added simultaneously .
	manualset3
115969	1	403609	13	NULL	NULL	0	NULL	MHC B haplotypes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the MHC B and Rfp-Y haplotypes segregating in broiler chickens are poorly documented .
	manualset3
115970	2	403609	13	NULL	NULL	0	NULL	Rfp-Y haplotypes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the MHC B and Rfp-Y haplotypes segregating in broiler chickens are poorly documented .
	manualset3
115971	3	403609	13	NULL	NULL	0	NULL	broiler chickens 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the MHC B and Rfp-Y haplotypes segregating in broiler chickens are poorly documented .
	manualset3
115972	1	403610	13	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the age-dependent increase and decline in IGF-I and IGFBP-3 were maintained in these supplemented animals .
	manualset3
115973	2	403610	13	NULL	NULL	0	NULL	decline	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the age-dependent increase and decline in IGF-I and IGFBP-3 were maintained in these supplemented animals .
	manualset3
115974	3	403610	13	NULL	NULL	0	NULL	IGF-I 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the age-dependent increase and decline in IGF-I and IGFBP-3 were maintained in these supplemented animals .
	manualset3
115975	4	403610	13	NULL	NULL	0	NULL	IGFBP-3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the age-dependent increase and decline in IGF-I and IGFBP-3 were maintained in these supplemented animals .
	manualset3
115976	5	403610	13	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the age-dependent increase and decline in IGF-I and IGFBP-3 were maintained in these supplemented animals .
	manualset3
115977	1	403611	13	NULL	NULL	0	NULL	measures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the considerable overlap on these measures between those who will develop PTSD , and those who eventually recover spontaneously , belies any attempt to identify any single or pathognomonic biological marker for risk .
	manualset3
115978	2	403611	13	NULL	NULL	0	NULL	PTSD	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the considerable overlap on these measures between those who will develop PTSD , and those who eventually recover spontaneously , belies any attempt to identify any single or pathognomonic biological marker for risk .
	manualset3
115979	3	403611	13	NULL	NULL	0	NULL	attempt	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the considerable overlap on these measures between those who will develop PTSD , and those who eventually recover spontaneously , belies any attempt to identify any single or pathognomonic biological marker for risk .
	manualset3
115980	4	403611	13	NULL	NULL	0	NULL	pathognomonic biological marker	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the considerable overlap on these measures between those who will develop PTSD , and those who eventually recover spontaneously , belies any attempt to identify any single or pathognomonic biological marker for risk .
	manualset3
115981	5	403611	13	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the considerable overlap on these measures between those who will develop PTSD , and those who eventually recover spontaneously , belies any attempt to identify any single or pathognomonic biological marker for risk .
	manualset3
115982	1	403612	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the expression of slow SM2 isoform in myotubes formed from slow ALD myoblasts only occurred when myoblasts were cultured in the presence of embryonic spinal cord .
	manualset3
115983	2	403612	13	NULL	NULL	NULL	NULL	slow SM2 isoform 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nevertheless , the expression of slow SM2 isoform in myotubes formed from slow ALD myoblasts only occurred when myoblasts were cultured in the presence of embryonic spinal cord .
	manualset3
115984	3	403612	13	NULL	NULL	0	NULL	myotubes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the expression of slow SM2 isoform in myotubes formed from slow ALD myoblasts only occurred when myoblasts were cultured in the presence of embryonic spinal cord .
	manualset3
115985	4	403612	13	NULL	NULL	0	NULL	slow ALD myoblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the expression of slow SM2 isoform in myotubes formed from slow ALD myoblasts only occurred when myoblasts were cultured in the presence of embryonic spinal cord .
	manualset3
115986	5	403612	13	NULL	NULL	0	NULL	myoblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the expression of slow SM2 isoform in myotubes formed from slow ALD myoblasts only occurred when myoblasts were cultured in the presence of embryonic spinal cord .
	manualset3
115987	6	403612	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the expression of slow SM2 isoform in myotubes formed from slow ALD myoblasts only occurred when myoblasts were cultured in the presence of embryonic spinal cord .
	manualset3
115988	7	403612	13	NULL	NULL	0	NULL	embryonic spinal cord	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the expression of slow SM2 isoform in myotubes formed from slow ALD myoblasts only occurred when myoblasts were cultured in the presence of embryonic spinal cord .
	manualset3
115989	1	403613	13	NULL	NULL	0	NULL	fold increase 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the fold increase in the lung accumulation of IRQ-PEG-LP , compared to the PEG-LP ( approximately 20-folds ) was substantially higher than other tissues ( & lt ; 5-fold ) .
	manualset3
115990	2	403613	13	NULL	NULL	0	NULL	lung accumulation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the fold increase in the lung accumulation of IRQ-PEG-LP , compared to the PEG-LP ( approximately 20-folds ) was substantially higher than other tissues ( & lt ; 5-fold ) .
	manualset3
115991	3	403613	13	NULL	NULL	0	NULL	IRQ-PEG-LP	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the fold increase in the lung accumulation of IRQ-PEG-LP , compared to the PEG-LP ( approximately 20-folds ) was substantially higher than other tissues ( & lt ; 5-fold ) .
	manualset3
115992	4	403613	13	NULL	NULL	0	NULL	PEG-LP	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the fold increase in the lung accumulation of IRQ-PEG-LP , compared to the PEG-LP ( approximately 20-folds ) was substantially higher than other tissues ( & lt ; 5-fold ) .
	manualset3
115993	5	403613	13	NULL	NULL	0	NULL	approximately 20-folds	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the fold increase in the lung accumulation of IRQ-PEG-LP , compared to the PEG-LP ( approximately 20-folds ) was substantially higher than other tissues ( & lt ; 5-fold ) .
	manualset3
115994	6	403613	13	NULL	NULL	0	NULL	tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the fold increase in the lung accumulation of IRQ-PEG-LP , compared to the PEG-LP ( approximately 20-folds ) was substantially higher than other tissues ( & lt ; 5-fold ) .
	manualset3
115995	7	403613	13	NULL	NULL	0	NULL	& lt ; 5-fold	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the fold increase in the lung accumulation of IRQ-PEG-LP , compared to the PEG-LP ( approximately 20-folds ) was substantially higher than other tissues ( & lt ; 5-fold ) .
	manualset3
115996	1	403614	13	NULL	NULL	0	NULL	gap	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the gap between science and practice may never be fully closed but will always have irresolvable conflicts that can only be contained .
	manualset3
115997	2	403614	13	NULL	NULL	0	NULL	science 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the gap between science and practice may never be fully closed but will always have irresolvable conflicts that can only be contained .
	manualset3
115998	3	403614	13	NULL	NULL	0	NULL	practice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the gap between science and practice may never be fully closed but will always have irresolvable conflicts that can only be contained .
	manualset3
115999	4	403614	13	NULL	NULL	0	NULL	irresolvable conflicts 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the gap between science and practice may never be fully closed but will always have irresolvable conflicts that can only be contained .
	manualset3
116000	1	403615	13	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the relationship between macroscopic properties ( pressure drop , treatment efficiency ) and microstructure can be assessed thanks to suitable structure modelling theories .
	manualset3
116001	2	403615	13	NULL	NULL	0	NULL	macroscopic properties	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the relationship between macroscopic properties ( pressure drop , treatment efficiency ) and microstructure can be assessed thanks to suitable structure modelling theories .
	manualset3
116002	3	403615	13	NULL	NULL	0	NULL	pressure drop	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the relationship between macroscopic properties ( pressure drop , treatment efficiency ) and microstructure can be assessed thanks to suitable structure modelling theories .
	manualset3
116003	4	403615	13	NULL	NULL	0	NULL	treatment efficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the relationship between macroscopic properties ( pressure drop , treatment efficiency ) and microstructure can be assessed thanks to suitable structure modelling theories .
	manualset3
116004	5	403615	13	NULL	NULL	0	NULL	microstructure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the relationship between macroscopic properties ( pressure drop , treatment efficiency ) and microstructure can be assessed thanks to suitable structure modelling theories .
	manualset3
116005	6	403615	13	NULL	NULL	0	NULL	thanks 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the relationship between macroscopic properties ( pressure drop , treatment efficiency ) and microstructure can be assessed thanks to suitable structure modelling theories .
	manualset3
116006	7	403615	13	NULL	NULL	0	NULL	structure modelling theories 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , the relationship between macroscopic properties ( pressure drop , treatment efficiency ) and microstructure can be assessed thanks to suitable structure modelling theories .
	manualset3
116007	1	403616	13	NULL	NULL	0	NULL	comparative studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , there have been no comparative studies of the activities and depth activity of several proteases in the SC on different body sites and at different times of the year .
	manualset3
116008	2	403616	13	NULL	NULL	0	NULL	activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , there have been no comparative studies of the activities and depth activity of several proteases in the SC on different body sites and at different times of the year .
	manualset3
116009	3	403616	13	NULL	NULL	0	NULL	depth activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , there have been no comparative studies of the activities and depth activity of several proteases in the SC on different body sites and at different times of the year .
	manualset3
116010	4	403616	13	NULL	NULL	0	NULL	proteases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , there have been no comparative studies of the activities and depth activity of several proteases in the SC on different body sites and at different times of the year .
	manualset3
116011	5	403616	13	NULL	NULL	0	NULL	SC 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , there have been no comparative studies of the activities and depth activity of several proteases in the SC on different body sites and at different times of the year .
	manualset3
116012	6	403616	13	NULL	NULL	0	NULL	body sites 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , there have been no comparative studies of the activities and depth activity of several proteases in the SC on different body sites and at different times of the year .
	manualset3
116013	7	403616	13	NULL	NULL	0	NULL	times	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , there have been no comparative studies of the activities and depth activity of several proteases in the SC on different body sites and at different times of the year .
	manualset3
116014	8	403616	13	NULL	NULL	0	NULL	year 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , there have been no comparative studies of the activities and depth activity of several proteases in the SC on different body sites and at different times of the year .
	manualset3
116015	1	403617	13	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , these findings support the concept that activation of thalamic nuclei will enhance DA function in a variety of forebrain areas in the rat .
	manualset3
116016	2	403617	13	NULL	NULL	0	NULL	concept	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , these findings support the concept that activation of thalamic nuclei will enhance DA function in a variety of forebrain areas in the rat .
	manualset3
116017	3	403617	13	NULL	NULL	0	NULL	activation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , these findings support the concept that activation of thalamic nuclei will enhance DA function in a variety of forebrain areas in the rat .
	manualset3
116018	4	403617	13	NULL	NULL	0	NULL	thalamic nuclei	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , these findings support the concept that activation of thalamic nuclei will enhance DA function in a variety of forebrain areas in the rat .
	manualset3
116019	5	403617	13	NULL	NULL	0	NULL	DA function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , these findings support the concept that activation of thalamic nuclei will enhance DA function in a variety of forebrain areas in the rat .
	manualset3
116020	6	403617	13	NULL	NULL	0	NULL	variety of forebrain areas 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , these findings support the concept that activation of thalamic nuclei will enhance DA function in a variety of forebrain areas in the rat .
	manualset3
116021	7	403617	13	NULL	NULL	0	NULL	rat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , these findings support the concept that activation of thalamic nuclei will enhance DA function in a variety of forebrain areas in the rat .
	manualset3
116022	1	403618	13	NULL	NULL	0	NULL	 sorting 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , when purified by sorting , T cells and non-B , non-T ( NBNT ) populations produced similar amounts of IL-4 in response to parasite antigen .
	manualset3
116023	2	403618	13	NULL	NULL	0	NULL	T cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , when purified by sorting , T cells and non-B , non-T ( NBNT ) populations produced similar amounts of IL-4 in response to parasite antigen .
	manualset3
116024	3	403618	13	NULL	NULL	0	NULL	non-B populations	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , when purified by sorting , T cells and non-B , non-T ( NBNT ) populations produced similar amounts of IL-4 in response to parasite antigen .
	manualset3
116025	4	403618	13	NULL	NULL	0	NULL	non-T ( NBNT ) populations	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , when purified by sorting , T cells and non-B , non-T ( NBNT ) populations produced similar amounts of IL-4 in response to parasite antigen .
	manualset3
116026	5	403618	13	NULL	NULL	0	NULL	amounts 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , when purified by sorting , T cells and non-B , non-T ( NBNT ) populations produced similar amounts of IL-4 in response to parasite antigen .
	manualset3
116027	6	403618	13	NULL	NULL	0	NULL	IL-4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , when purified by sorting , T cells and non-B , non-T ( NBNT ) populations produced similar amounts of IL-4 in response to parasite antigen .
	manualset3
116028	7	403618	13	NULL	NULL	0	NULL	response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , when purified by sorting , T cells and non-B , non-T ( NBNT ) populations produced similar amounts of IL-4 in response to parasite antigen .
	manualset3
116029	8	403618	13	NULL	NULL	0	NULL	parasite antigen	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevertheless , when purified by sorting , T cells and non-B , non-T ( NBNT ) populations produced similar amounts of IL-4 in response to parasite antigen .
	manualset3
116030	1	403619	13	NULL	NULL	0	NULL	Nevirapine nanosuspensions 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevirapine nanosuspensions for HIV reservoir targeting .
	manualset3
116031	2	403619	13	NULL	NULL	0	NULL	 HIV reservoir targeting 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Nevirapine nanosuspensions for HIV reservoir targeting .
	manualset3
116032	1	403620	13	NULL	NULL	0	NULL	New agents 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	New agents active against Mycobacterium avium complex selected by molecular topology : a virtual screening method .
	manualset3
116033	2	403620	13	NULL	NULL	0	NULL	Mycobacterium avium complex 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	New agents active against Mycobacterium avium complex selected by molecular topology : a virtual screening method .
	manualset3
116034	3	403620	13	NULL	NULL	0	NULL	molecular topology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	New agents active against Mycobacterium avium complex selected by molecular topology : a virtual screening method .
	manualset3
116035	4	403620	13	NULL	NULL	0	NULL	virtual screening method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	New agents active against Mycobacterium avium complex selected by molecular topology : a virtual screening method .
	manualset3
116036	1	403621	13	NULL	NULL	0	NULL	New analogs of curcumin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	New analogs of curcumin with improved properties are needed to meet therapeutic requirements .
	manualset3
116037	2	403621	13	NULL	NULL	0	NULL	properties	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	New analogs of curcumin with improved properties are needed to meet therapeutic requirements .
	manualset3
116038	3	403621	13	NULL	NULL	0	NULL	therapeutic requirements	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	New analogs of curcumin with improved properties are needed to meet therapeutic requirements .
	manualset3
116039	1	403622	13	NULL	NULL	0	NULL	New archival documentation	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	New archival documentation now demonstrates that Le Bon exercised significant influence on U.S. military thinking and practice through World War II .
	manualset3
116040	2	403622	13	NULL	NULL	0	NULL	Le Bon	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	New archival documentation now demonstrates that Le Bon exercised significant influence on U.S. military thinking and practice through World War II .
	manualset3
116041	3	403622	13	NULL	NULL	0	NULL	influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	New archival documentation now demonstrates that Le Bon exercised significant influence on U.S. military thinking and practice through World War II .
	manualset3
116042	4	403622	13	NULL	NULL	0	NULL	U.S. military 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	New archival documentation now demonstrates that Le Bon exercised significant influence on U.S. military thinking and practice through World War II .
	manualset3
116043	5	403622	13	NULL	NULL	0	NULL	thinking	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	New archival documentation now demonstrates that Le Bon exercised significant influence on U.S. military thinking and practice through World War II .
	manualset3
116044	6	403622	13	NULL	NULL	0	NULL	practice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	New archival documentation now demonstrates that Le Bon exercised significant influence on U.S. military thinking and practice through World War II .
	manualset3
116045	7	403622	13	NULL	NULL	0	NULL	World War II	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	New archival documentation now demonstrates that Le Bon exercised significant influence on U.S. military thinking and practice through World War II .
	manualset3
116046	1	403623	13	NULL	NULL	0	NULL	New extracellular resistance mechanism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	New extracellular resistance mechanism for cisplatin .
	manualset3
116047	2	403623	13	NULL	NULL	0	NULL	cisplatin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	New extracellular resistance mechanism for cisplatin .
	manualset3
116048	1	403624	13	NULL	NULL	0	NULL	New formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	New formation of smooth muscle in the lung .
	manualset3
116049	2	403624	13	NULL	NULL	NULL	NULL	smooth muscle	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	New formation of smooth muscle in the lung .
	manualset3
116050	3	403624	13	NULL	NULL	0	NULL	lung	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	New formation of smooth muscle in the lung .
	manualset3
116051	1	403625	13	NULL	NULL	0	NULL	New insights	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	New insights into diffusion in 3D crowded media by Monte Carlo simulations : effect of size , mobility and spatial distribution of obstacles .
	manualset3
116052	2	403625	13	NULL	NULL	0	NULL	diffusion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	New insights into diffusion in 3D crowded media by Monte Carlo simulations : effect of size , mobility and spatial distribution of obstacles .
	manualset3
116053	3	403625	13	NULL	NULL	0	NULL	3D crowded media 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	New insights into diffusion in 3D crowded media by Monte Carlo simulations : effect of size , mobility and spatial distribution of obstacles .
	manualset3
116054	4	403625	13	NULL	NULL	0	NULL	Monte Carlo simulations 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	New insights into diffusion in 3D crowded media by Monte Carlo simulations : effect of size , mobility and spatial distribution of obstacles .
	manualset3
116055	5	403625	13	NULL	NULL	0	NULL	effect of size	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	New insights into diffusion in 3D crowded media by Monte Carlo simulations : effect of size , mobility and spatial distribution of obstacles .
	manualset3
116056	6	403625	13	NULL	NULL	0	NULL	effect of mobility	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	New insights into diffusion in 3D crowded media by Monte Carlo simulations : effect of size , mobility and spatial distribution of obstacles .
	manualset3
116057	7	403625	13	NULL	NULL	0	NULL	effect of spatial distribution 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	New insights into diffusion in 3D crowded media by Monte Carlo simulations : effect of size , mobility and spatial distribution of obstacles .
	manualset3
116058	8	403625	13	NULL	NULL	0	NULL	obstacles 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	New insights into diffusion in 3D crowded media by Monte Carlo simulations : effect of size , mobility and spatial distribution of obstacles .
	manualset3
116059	1	403626	13	NULL	NULL	0	NULL	New insights	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	New insights into renal transplantation .
	manualset3
116060	2	403626	13	NULL	NULL	0	NULL	renal transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	New insights into renal transplantation .
	manualset3
116061	1	403627	13	NULL	NULL	0	NULL	New insights 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	New insights into the roles of megalin/LRP2 and the regulation of its functional expression .
	manualset3
116062	2	403627	13	NULL	NULL	0	NULL	roles	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	New insights into the roles of megalin/LRP2 and the regulation of its functional expression .
	manualset3
116063	3	403627	13	NULL	NULL	0	NULL	megalin/LRP2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	New insights into the roles of megalin/LRP2 and the regulation of its functional expression .
	manualset3
116064	4	403627	13	NULL	NULL	0	NULL	regulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	New insights into the roles of megalin/LRP2 and the regulation of its functional expression .
	manualset3
116065	5	403627	13	NULL	NULL	0	NULL	functional expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	New insights into the roles of megalin/LRP2 and the regulation of its functional expression .
	manualset3
116066	1	403628	13	NULL	NULL	0	NULL	New insights	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	New insights into the target site and mode of action of the antifungal protein of Aspergillus giganteus .
	manualset3
116067	2	403628	13	NULL	NULL	0	NULL	target site	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	New insights into the target site and mode of action of the antifungal protein of Aspergillus giganteus .
	manualset3
116068	3	403628	13	NULL	NULL	0	NULL	mode of action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	New insights into the target site and mode of action of the antifungal protein of Aspergillus giganteus .
	manualset3
116069	4	403628	13	NULL	NULL	0	NULL	antifungal protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	New insights into the target site and mode of action of the antifungal protein of Aspergillus giganteus .
	manualset3
116070	5	403628	13	NULL	NULL	0	NULL	Aspergillus giganteus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	New insights into the target site and mode of action of the antifungal protein of Aspergillus giganteus .
	manualset3
116071	1	403629	13	NULL	NULL	0	NULL	New ligands 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	New ligands 1 , 1 , 1-tris ( diphenylphosphinomethyl ) ethane ( CH3C ( CH2PPh2 ) 3 ) 1 and 1 , 1 , 1-tris - ( diphenylphosphino methyl ) ethane trisulphide ( CH3C ( CH2P ( S ) Ph2 ) 3 ) 2 for stabilization of Au ( degrees ) - nanoparticles having small core diameter were prepared .
	manualset3
116072	2	403629	13	NULL	NULL	0	NULL	1 , 1 , 1-tris ( diphenylphosphinomethyl ) ethane ( CH3C ( CH2PPh2 ) 3 ) 1 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	New ligands 1 , 1 , 1-tris ( diphenylphosphinomethyl ) ethane ( CH3C ( CH2PPh2 ) 3 ) 1 and 1 , 1 , 1-tris - ( diphenylphosphino methyl ) ethane trisulphide ( CH3C ( CH2P ( S ) Ph2 ) 3 ) 2 for stabilization of Au ( degrees ) - nanoparticles having small core diameter were prepared .
	manualset3
116073	3	403629	13	NULL	NULL	0	NULL	1 , 1 , 1-tris - ( diphenylphosphino methyl ) ethane trisulphide ( CH3C ( CH2P ( S ) Ph2 ) 3 ) 2 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	New ligands 1 , 1 , 1-tris ( diphenylphosphinomethyl ) ethane ( CH3C ( CH2PPh2 ) 3 ) 1 and 1 , 1 , 1-tris - ( diphenylphosphino methyl ) ethane trisulphide ( CH3C ( CH2P ( S ) Ph2 ) 3 ) 2 for stabilization of Au ( degrees ) - nanoparticles having small core diameter were prepared .
	manualset3
116074	4	403629	13	NULL	NULL	0	NULL	stabilization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	New ligands 1 , 1 , 1-tris ( diphenylphosphinomethyl ) ethane ( CH3C ( CH2PPh2 ) 3 ) 1 and 1 , 1 , 1-tris - ( diphenylphosphino methyl ) ethane trisulphide ( CH3C ( CH2P ( S ) Ph2 ) 3 ) 2 for stabilization of Au ( degrees ) - nanoparticles having small core diameter were prepared .
	manualset3
116075	5	403629	13	NULL	NULL	0	NULL	Au ( degrees ) - nanoparticles	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	New ligands 1 , 1 , 1-tris ( diphenylphosphinomethyl ) ethane ( CH3C ( CH2PPh2 ) 3 ) 1 and 1 , 1 , 1-tris - ( diphenylphosphino methyl ) ethane trisulphide ( CH3C ( CH2P ( S ) Ph2 ) 3 ) 2 for stabilization of Au ( degrees ) - nanoparticles having small core diameter were prepared .
	manualset3
116076	6	403629	13	NULL	NULL	0	NULL	small core diameter	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	New ligands 1 , 1 , 1-tris ( diphenylphosphinomethyl ) ethane ( CH3C ( CH2PPh2 ) 3 ) 1 and 1 , 1 , 1-tris - ( diphenylphosphino methyl ) ethane trisulphide ( CH3C ( CH2P ( S ) Ph2 ) 3 ) 2 for stabilization of Au ( degrees ) - nanoparticles having small core diameter were prepared .
	manualset3
116077	1	403630	13	NULL	NULL	0	NULL	New mechanism	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	New mechanism of plasmid curing by psychotropic drugs .
	manualset3
116078	2	403630	13	NULL	NULL	0	NULL	plasmid curing 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	New mechanism of plasmid curing by psychotropic drugs .
	manualset3
116079	3	403630	13	NULL	NULL	0	NULL	psychotropic drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	New mechanism of plasmid curing by psychotropic drugs .
	manualset3
116080	1	403631	13	NULL	NULL	0	NULL	New parameters 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	New parameters to monitor the progression of diabetic nephropathy .
	manualset3
116081	2	403631	13	NULL	NULL	0	NULL	monitor 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	New parameters to monitor the progression of diabetic nephropathy .
	manualset3
116082	3	403631	13	NULL	NULL	0	NULL	progression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	New parameters to monitor the progression of diabetic nephropathy .
	manualset3
116083	4	403631	13	NULL	NULL	0	NULL	diabetic nephropathy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	New parameters to monitor the progression of diabetic nephropathy .
	manualset3
116084	1	403632	13	NULL	NULL	0	NULL	New pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	New pathways of phagocyte activation : the coupling of receptor-linked phospholipase D and the role of tyrosine kinase in primed neutrophils .
	manualset3
116085	2	403632	13	NULL	NULL	0	NULL	phagocyte activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	New pathways of phagocyte activation : the coupling of receptor-linked phospholipase D and the role of tyrosine kinase in primed neutrophils .
	manualset3
116086	3	403632	13	NULL	NULL	0	NULL	coupling 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	New pathways of phagocyte activation : the coupling of receptor-linked phospholipase D and the role of tyrosine kinase in primed neutrophils .
	manualset3
116087	4	403632	13	NULL	NULL	0	NULL	receptor-linked phospholipase D	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	New pathways of phagocyte activation : the coupling of receptor-linked phospholipase D and the role of tyrosine kinase in primed neutrophils .
	manualset3
116088	5	403632	13	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	New pathways of phagocyte activation : the coupling of receptor-linked phospholipase D and the role of tyrosine kinase in primed neutrophils .
	manualset3
116089	6	403632	13	NULL	NULL	0	NULL	tyrosine kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	New pathways of phagocyte activation : the coupling of receptor-linked phospholipase D and the role of tyrosine kinase in primed neutrophils .
	manualset3
116090	7	403632	13	NULL	NULL	0	NULL	neutrophils	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	New pathways of phagocyte activation : the coupling of receptor-linked phospholipase D and the role of tyrosine kinase in primed neutrophils .
	manualset3
116091	1	403633	13	NULL	NULL	0	NULL	New phenotypes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	New phenotypes associated with mucAB : alteration of a MucA sequence homologous to the LexA cleavage site .
	manualset3
116092	2	403633	13	NULL	NULL	0	NULL	mucAB	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	New phenotypes associated with mucAB : alteration of a MucA sequence homologous to the LexA cleavage site .
	manualset3
116093	3	403633	13	NULL	NULL	0	NULL	alteration	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	New phenotypes associated with mucAB : alteration of a MucA sequence homologous to the LexA cleavage site .
	manualset3
116094	4	403633	13	NULL	NULL	NULL	NULL	MucA sequence	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	New phenotypes associated with mucAB : alteration of a MucA sequence homologous to the LexA cleavage site .
	manualset3
116095	5	403633	13	NULL	NULL	0	NULL	LexA cleavage site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	New phenotypes associated with mucAB : alteration of a MucA sequence homologous to the LexA cleavage site .
	manualset3
116096	1	403634	13	NULL	NULL	0	NULL	New procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	New procedure for stabilization of lesser metatarsophalangeal joints : a preliminary study .
	manualset3
116097	2	403634	13	NULL	NULL	0	NULL	stabilization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	New procedure for stabilization of lesser metatarsophalangeal joints : a preliminary study .
	manualset3
116098	3	403634	13	NULL	NULL	0	NULL	metatarsophalangeal joints 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	New procedure for stabilization of lesser metatarsophalangeal joints : a preliminary study .
	manualset3
116099	4	403634	13	NULL	NULL	0	NULL	preliminary study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	New procedure for stabilization of lesser metatarsophalangeal joints : a preliminary study .
	manualset3
116100	1	403635	13	NULL	NULL	NULL	NULL	New provider responsibilities	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	New provider responsibilities under the Patient Self-Determination Act : living wills , durable powers of attorney , and the law .
	manualset3
116101	2	403635	13	NULL	NULL	0	NULL	Patient Self-Determination Act	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	New provider responsibilities under the Patient Self-Determination Act : living wills , durable powers of attorney , and the law .
	manualset3
116102	3	403635	13	NULL	NULL	0	NULL	living wills	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	New provider responsibilities under the Patient Self-Determination Act : living wills , durable powers of attorney , and the law .
	manualset3
116103	4	403635	13	NULL	NULL	0	NULL	durable powers of attorney	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	New provider responsibilities under the Patient Self-Determination Act : living wills , durable powers of attorney , and the law .
	manualset3
116104	5	403635	13	NULL	NULL	0	NULL	law	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	New provider responsibilities under the Patient Self-Determination Act : living wills , durable powers of attorney , and the law .
	manualset3
116105	1	403636	13	NULL	NULL	0	NULL	New rapid phenotypic assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	New rapid phenotypic assays for the detection of rifampin resistance in Mycobacterium tuberculosis have recently been described , but most of these require liquid cultures , which reduces the utility of many tests in terms of turnaround times .
	manualset3
116106	2	403636	13	NULL	NULL	0	NULL	detection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	New rapid phenotypic assays for the detection of rifampin resistance in Mycobacterium tuberculosis have recently been described , but most of these require liquid cultures , which reduces the utility of many tests in terms of turnaround times .
	manualset3
116107	3	403636	13	NULL	NULL	0	NULL	rifampin resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	New rapid phenotypic assays for the detection of rifampin resistance in Mycobacterium tuberculosis have recently been described , but most of these require liquid cultures , which reduces the utility of many tests in terms of turnaround times .
	manualset3
116108	4	403636	13	NULL	NULL	0	NULL	Mycobacterium tuberculosis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	New rapid phenotypic assays for the detection of rifampin resistance in Mycobacterium tuberculosis have recently been described , but most of these require liquid cultures , which reduces the utility of many tests in terms of turnaround times .
	manualset3
116109	5	403636	13	NULL	NULL	0	NULL	liquid cultures	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	New rapid phenotypic assays for the detection of rifampin resistance in Mycobacterium tuberculosis have recently been described , but most of these require liquid cultures , which reduces the utility of many tests in terms of turnaround times .
	manualset3
116110	6	403636	13	NULL	NULL	0	NULL	utility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	New rapid phenotypic assays for the detection of rifampin resistance in Mycobacterium tuberculosis have recently been described , but most of these require liquid cultures , which reduces the utility of many tests in terms of turnaround times .
	manualset3
116111	7	403636	13	NULL	NULL	0	NULL	tests	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	New rapid phenotypic assays for the detection of rifampin resistance in Mycobacterium tuberculosis have recently been described , but most of these require liquid cultures , which reduces the utility of many tests in terms of turnaround times .
	manualset3
116112	8	403636	13	NULL	NULL	NULL	NULL	turnaround times	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	New rapid phenotypic assays for the detection of rifampin resistance in Mycobacterium tuberculosis have recently been described , but most of these require liquid cultures , which reduces the utility of many tests in terms of turnaround times .
	manualset3
116113	1	403637	13	NULL	NULL	0	NULL	New solutions 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	New solutions clean and disinfect ceilings at medical facilities .
	manualset3
116114	2	403637	13	NULL	NULL	0	NULL	ceilings	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	New solutions clean and disinfect ceilings at medical facilities .
	manualset3
116115	3	403637	13	NULL	NULL	0	NULL	medical facilities	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	New solutions clean and disinfect ceilings at medical facilities .
	manualset3
116116	1	403638	13	NULL	NULL	0	NULL	New vascular graft	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	New vascular graft for simplification of the aortic valve reimplantation technique .
	manualset3
116117	2	403638	13	NULL	NULL	0	NULL	simplification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	New vascular graft for simplification of the aortic valve reimplantation technique .
	manualset3
116118	3	403638	13	NULL	NULL	0	NULL	aortic valve reimplantation technique	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	New vascular graft for simplification of the aortic valve reimplantation technique .
	manualset3
116119	1	403639	13	NULL	NULL	0	NULL	New vesicular ampicillin-loaded delivery systems	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	New vesicular ampicillin-loaded delivery systems for topical application : characterization , in vitro permeation experiments and antimicrobial activity .
	manualset3
116120	2	403639	13	NULL	NULL	0	NULL	topical application	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	New vesicular ampicillin-loaded delivery systems for topical application : characterization , in vitro permeation experiments and antimicrobial activity .
	manualset3
116121	3	403639	13	NULL	NULL	0	NULL	characterization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	New vesicular ampicillin-loaded delivery systems for topical application : characterization , in vitro permeation experiments and antimicrobial activity .
	manualset3
116122	4	403639	13	NULL	NULL	0	NULL	in vitro permeation experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	New vesicular ampicillin-loaded delivery systems for topical application : characterization , in vitro permeation experiments and antimicrobial activity .
	manualset3
116123	5	403639	13	NULL	NULL	0	NULL	antimicrobial activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	New vesicular ampicillin-loaded delivery systems for topical application : characterization , in vitro permeation experiments and antimicrobial activity .
	manualset3
116124	1	403640	13	NULL	NULL	0	NULL	New data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	New data show that national family planning programs have made impressive progress in the last 25 years .
	manualset3
116125	2	403640	13	NULL	NULL	0	NULL	national family planning programs	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	New data show that national family planning programs have made impressive progress in the last 25 years .
	manualset3
116126	3	403640	13	NULL	NULL	0	NULL	impressive progress	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	New data show that national family planning programs have made impressive progress in the last 25 years .
	manualset3
116127	4	403640	13	NULL	NULL	0	NULL	last 25 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	New data show that national family planning programs have made impressive progress in the last 25 years .
	manualset3
116128	1	403641	13	NULL	NULL	0	NULL	New insights	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	New insights are emerging into the role of the megakaryocytopoiesis regulator thrombopoietin ( TPO ) and its receptor , c-Mpl , in ET and related disorders , but TPO-Mpl dynamics appear to be complex .
	manualset3
116129	2	403641	13	NULL	NULL	0	NULL	role 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	New insights are emerging into the role of the megakaryocytopoiesis regulator thrombopoietin ( TPO ) and its receptor , c-Mpl , in ET and related disorders , but TPO-Mpl dynamics appear to be complex .
	manualset3
116130	3	403641	13	NULL	NULL	0	NULL	megakaryocytopoiesis regulator thrombopoietin ( TPO ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	New insights are emerging into the role of the megakaryocytopoiesis regulator thrombopoietin ( TPO ) and its receptor , c-Mpl , in ET and related disorders , but TPO-Mpl dynamics appear to be complex .
	manualset3
116131	4	403641	13	NULL	NULL	0	NULL	receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	New insights are emerging into the role of the megakaryocytopoiesis regulator thrombopoietin ( TPO ) and its receptor , c-Mpl , in ET and related disorders , but TPO-Mpl dynamics appear to be complex .
	manualset3
116132	5	403641	13	NULL	NULL	0	NULL	c-Mpl	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	New insights are emerging into the role of the megakaryocytopoiesis regulator thrombopoietin ( TPO ) and its receptor , c-Mpl , in ET and related disorders , but TPO-Mpl dynamics appear to be complex .
	manualset3
116133	6	403641	13	NULL	NULL	0	NULL	ET 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	New insights are emerging into the role of the megakaryocytopoiesis regulator thrombopoietin ( TPO ) and its receptor , c-Mpl , in ET and related disorders , but TPO-Mpl dynamics appear to be complex .
	manualset3
116134	7	403641	13	NULL	NULL	0	NULL	disorders 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	New insights are emerging into the role of the megakaryocytopoiesis regulator thrombopoietin ( TPO ) and its receptor , c-Mpl , in ET and related disorders , but TPO-Mpl dynamics appear to be complex .
	manualset3
116135	8	403641	13	NULL	NULL	0	NULL	TPO-Mpl dynamics 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	New insights are emerging into the role of the megakaryocytopoiesis regulator thrombopoietin ( TPO ) and its receptor , c-Mpl , in ET and related disorders , but TPO-Mpl dynamics appear to be complex .
	manualset3
116136	1	403642	13	NULL	NULL	0	NULL	New probes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	New probes , designed to delineate the individual contributions of the fasciculin residues to the complex formation and conformation , were generated by site-directed mutagenesis of a synthetic Fas2 gene .
	manualset3
116137	2	403642	13	NULL	NULL	0	NULL	contributions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	New probes , designed to delineate the individual contributions of the fasciculin residues to the complex formation and conformation , were generated by site-directed mutagenesis of a synthetic Fas2 gene .
	manualset3
116138	3	403642	13	NULL	NULL	0	NULL	fasciculin residues 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	New probes , designed to delineate the individual contributions of the fasciculin residues to the complex formation and conformation , were generated by site-directed mutagenesis of a synthetic Fas2 gene .
	manualset3
116139	4	403642	13	NULL	NULL	0	NULL	complex formation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	New probes , designed to delineate the individual contributions of the fasciculin residues to the complex formation and conformation , were generated by site-directed mutagenesis of a synthetic Fas2 gene .
	manualset3
116140	5	403642	13	NULL	NULL	0	NULL	conformation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	New probes , designed to delineate the individual contributions of the fasciculin residues to the complex formation and conformation , were generated by site-directed mutagenesis of a synthetic Fas2 gene .
	manualset3
116141	6	403642	13	NULL	NULL	0	NULL	site-directed mutagenesis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	New probes , designed to delineate the individual contributions of the fasciculin residues to the complex formation and conformation , were generated by site-directed mutagenesis of a synthetic Fas2 gene .
	manualset3
116142	7	403642	13	NULL	NULL	0	NULL	Fas2 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	New probes , designed to delineate the individual contributions of the fasciculin residues to the complex formation and conformation , were generated by site-directed mutagenesis of a synthetic Fas2 gene .
	manualset3
116143	1	403643	13	NULL	NULL	0	NULL	New study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	New study fails to find link between MMR and autism .
	manualset3
116144	2	403643	13	NULL	NULL	0	NULL	link 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	New study fails to find link between MMR and autism .
	manualset3
116145	3	403643	13	NULL	NULL	0	NULL	MMR	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	New study fails to find link between MMR and autism .
	manualset3
116146	4	403643	13	NULL	NULL	0	NULL	autism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	New study fails to find link between MMR and autism .
	manualset3
116147	1	403644	13	NULL	NULL	0	NULL	New technology 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	New technology and new initiatives in U.S. workplace testing .
	manualset3
116148	2	403644	13	NULL	NULL	0	NULL	new initiatives 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	New technology and new initiatives in U.S. workplace testing .
	manualset3
116149	3	403644	13	NULL	NULL	0	NULL	U.S. workplace testing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	New technology and new initiatives in U.S. workplace testing .
	manualset3
116150	1	403645	13	NULL	NULL	0	NULL	New plan	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	New plan to promote information technology released to mostly good reviews , but concerns remain about its scope and funding .
	manualset3
116151	2	403645	13	NULL	NULL	0	NULL	information technology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	New plan to promote information technology released to mostly good reviews , but concerns remain about its scope and funding .
	manualset3
116152	3	403645	13	NULL	NULL	0	NULL	good reviews	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	New plan to promote information technology released to mostly good reviews , but concerns remain about its scope and funding .
	manualset3
116153	4	403645	13	NULL	NULL	0	NULL	concerns	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	New plan to promote information technology released to mostly good reviews , but concerns remain about its scope and funding .
	manualset3
116154	5	403645	13	NULL	NULL	0	NULL	scope	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	New plan to promote information technology released to mostly good reviews , but concerns remain about its scope and funding .
	manualset3
116155	6	403645	13	NULL	NULL	0	NULL	funding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	New plan to promote information technology released to mostly good reviews , but concerns remain about its scope and funding .
	manualset3
116156	1	403646	13	NULL	NULL	0	NULL	Newborn screening	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Newborn screening for inborn errors of metabolism in Beijing , China : 22 years of experience .
	manualset3
116157	2	403646	13	NULL	NULL	0	NULL	inborn errors of metabolism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Newborn screening for inborn errors of metabolism in Beijing , China : 22 years of experience .
	manualset3
116158	3	403646	13	NULL	NULL	0	NULL	Beijing	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Newborn screening for inborn errors of metabolism in Beijing , China : 22 years of experience .
	manualset3
116159	4	403646	13	NULL	NULL	0	NULL	China	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Newborn screening for inborn errors of metabolism in Beijing , China : 22 years of experience .
	manualset3
116160	5	403646	13	NULL	NULL	0	NULL	22 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Newborn screening for inborn errors of metabolism in Beijing , China : 22 years of experience .
	manualset3
116161	6	403646	13	NULL	NULL	0	NULL	experience 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Newborn screening for inborn errors of metabolism in Beijing , China : 22 years of experience .
	manualset3
116162	1	403647	13	NULL	NULL	0	NULL	Newer anticonvulsant drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Newer anticonvulsant drugs may offer additional management opportunities .
	manualset3
116163	2	403647	13	NULL	NULL	0	NULL	additional management opportunities 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Newer anticonvulsant drugs may offer additional management opportunities .
	manualset3
116164	1	403648	13	NULL	NULL	0	NULL	Newer management strategies 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Newer management strategies for these complications of pancreatic inflammatory disease are discussed , including percutaneous drainage of pseudocysts and the use of octreotide in the management of pancreatic ascites and pancreatic fistulas .
	manualset3
116165	2	403648	13	NULL	NULL	0	NULL	complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Newer management strategies for these complications of pancreatic inflammatory disease are discussed , including percutaneous drainage of pseudocysts and the use of octreotide in the management of pancreatic ascites and pancreatic fistulas .
	manualset3
116166	3	403648	13	NULL	NULL	0	NULL	pancreatic inflammatory disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Newer management strategies for these complications of pancreatic inflammatory disease are discussed , including percutaneous drainage of pseudocysts and the use of octreotide in the management of pancreatic ascites and pancreatic fistulas .
	manualset3
116167	4	403648	13	NULL	NULL	0	NULL	percutaneous drainage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Newer management strategies for these complications of pancreatic inflammatory disease are discussed , including percutaneous drainage of pseudocysts and the use of octreotide in the management of pancreatic ascites and pancreatic fistulas .
	manualset3
116168	5	403648	13	NULL	NULL	0	NULL	pseudocysts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Newer management strategies for these complications of pancreatic inflammatory disease are discussed , including percutaneous drainage of pseudocysts and the use of octreotide in the management of pancreatic ascites and pancreatic fistulas .
	manualset3
116169	6	403648	13	NULL	NULL	0	NULL	octreotide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Newer management strategies for these complications of pancreatic inflammatory disease are discussed , including percutaneous drainage of pseudocysts and the use of octreotide in the management of pancreatic ascites and pancreatic fistulas .
	manualset3
116170	7	403648	13	NULL	NULL	0	NULL	management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Newer management strategies for these complications of pancreatic inflammatory disease are discussed , including percutaneous drainage of pseudocysts and the use of octreotide in the management of pancreatic ascites and pancreatic fistulas .
	manualset3
116171	8	403648	13	NULL	NULL	0	NULL	pancreatic ascites	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Newer management strategies for these complications of pancreatic inflammatory disease are discussed , including percutaneous drainage of pseudocysts and the use of octreotide in the management of pancreatic ascites and pancreatic fistulas .
	manualset3
116172	9	403648	13	NULL	NULL	0	NULL	pancreatic fistulas 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Newer management strategies for these complications of pancreatic inflammatory disease are discussed , including percutaneous drainage of pseudocysts and the use of octreotide in the management of pancreatic ascites and pancreatic fistulas .
	manualset3
116173	1	403649	13	NULL	NULL	0	NULL	autosomal recessive faciothoracoskeletal syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Newly recognized autosomal recessive faciothoracoskeletal syndrome .
	manualset3
116174	1	403650	13	NULL	NULL	0	NULL	FACS-sorted VEGFR2 + cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , FACS-sorted VEGFR2 + cells expressed highest and lowest levels of SMC - and fibroblast-specific markers , respectively , at days 7-14 after retinoic acid ( RA ) as compared with VEGFR2 + / PDGFR + cells .
	manualset3
116175	2	403650	13	NULL	NULL	NULL	NULL	highest levels of SMC	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Next , FACS-sorted VEGFR2 + cells expressed highest and lowest levels of SMC - and fibroblast-specific markers , respectively , at days 7-14 after retinoic acid ( RA ) as compared with VEGFR2 + / PDGFR + cells .
	manualset3
116176	3	403650	13	NULL	NULL	NULL	NULL	lowest levels of fibroblast-specific markers 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Next , FACS-sorted VEGFR2 + cells expressed highest and lowest levels of SMC - and fibroblast-specific markers , respectively , at days 7-14 after retinoic acid ( RA ) as compared with VEGFR2 + / PDGFR + cells .
	manualset3
116177	4	403650	13	NULL	NULL	0	NULL	days 7-14 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , FACS-sorted VEGFR2 + cells expressed highest and lowest levels of SMC - and fibroblast-specific markers , respectively , at days 7-14 after retinoic acid ( RA ) as compared with VEGFR2 + / PDGFR + cells .
	manualset3
116178	5	403650	13	NULL	NULL	0	NULL	retinoic acid ( RA ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , FACS-sorted VEGFR2 + cells expressed highest and lowest levels of SMC - and fibroblast-specific markers , respectively , at days 7-14 after retinoic acid ( RA ) as compared with VEGFR2 + / PDGFR + cells .
	manualset3
116179	6	403650	13	NULL	NULL	0	NULL	VEGFR2 + / PDGFR + cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , FACS-sorted VEGFR2 + cells expressed highest and lowest levels of SMC - and fibroblast-specific markers , respectively , at days 7-14 after retinoic acid ( RA ) as compared with VEGFR2 + / PDGFR + cells .
	manualset3
116180	1	403651	13	NULL	NULL	0	NULL	1 : 1 mixture 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , a 1 : 1 mixture of glycerol monomethacrylate and glycerol dimethacrylate was used for hydrophilic surface modification , and it was added directly to the MIP for ( S ) - naproxen or - ibuprofen 4 h after the start of molecular imprinting .
	manualset3
116181	2	403651	13	NULL	NULL	0	NULL	glycerol monomethacrylate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , a 1 : 1 mixture of glycerol monomethacrylate and glycerol dimethacrylate was used for hydrophilic surface modification , and it was added directly to the MIP for ( S ) - naproxen or - ibuprofen 4 h after the start of molecular imprinting .
	manualset3
116182	3	403651	13	NULL	NULL	0	NULL	glycerol dimethacrylate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , a 1 : 1 mixture of glycerol monomethacrylate and glycerol dimethacrylate was used for hydrophilic surface modification , and it was added directly to the MIP for ( S ) - naproxen or - ibuprofen 4 h after the start of molecular imprinting .
	manualset3
116183	4	403651	13	NULL	NULL	0	NULL	hydrophilic surface modification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , a 1 : 1 mixture of glycerol monomethacrylate and glycerol dimethacrylate was used for hydrophilic surface modification , and it was added directly to the MIP for ( S ) - naproxen or - ibuprofen 4 h after the start of molecular imprinting .
	manualset3
116184	5	403651	13	NULL	NULL	0	NULL	MIP 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , a 1 : 1 mixture of glycerol monomethacrylate and glycerol dimethacrylate was used for hydrophilic surface modification , and it was added directly to the MIP for ( S ) - naproxen or - ibuprofen 4 h after the start of molecular imprinting .
	manualset3
116185	6	403651	13	NULL	NULL	0	NULL	( S ) - naproxen	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , a 1 : 1 mixture of glycerol monomethacrylate and glycerol dimethacrylate was used for hydrophilic surface modification , and it was added directly to the MIP for ( S ) - naproxen or - ibuprofen 4 h after the start of molecular imprinting .
	manualset3
116186	7	403651	13	NULL	NULL	0	NULL	ibuprofen 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , a 1 : 1 mixture of glycerol monomethacrylate and glycerol dimethacrylate was used for hydrophilic surface modification , and it was added directly to the MIP for ( S ) - naproxen or - ibuprofen 4 h after the start of molecular imprinting .
	manualset3
116187	8	403651	13	NULL	NULL	0	NULL	4 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , a 1 : 1 mixture of glycerol monomethacrylate and glycerol dimethacrylate was used for hydrophilic surface modification , and it was added directly to the MIP for ( S ) - naproxen or - ibuprofen 4 h after the start of molecular imprinting .
	manualset3
116188	9	403651	13	NULL	NULL	0	NULL	molecular imprinting	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , a 1 : 1 mixture of glycerol monomethacrylate and glycerol dimethacrylate was used for hydrophilic surface modification , and it was added directly to the MIP for ( S ) - naproxen or - ibuprofen 4 h after the start of molecular imprinting .
	manualset3
116189	1	403652	13	NULL	NULL	0	NULL	effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , the effects of restraint stress , nociceptive stimulus and acute inflammatory stress on the expression of the prolactin-releasing peptide mRNA in the dorsomedial hypothalamic nucleus , nucleus of the solitary tract and ventrolateral medulla were examined using in situ hybridization histochemistry for prolactin-releasing peptide mRNA .
	manualset3
116190	2	403652	13	NULL	NULL	0	NULL	restraint stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , the effects of restraint stress , nociceptive stimulus and acute inflammatory stress on the expression of the prolactin-releasing peptide mRNA in the dorsomedial hypothalamic nucleus , nucleus of the solitary tract and ventrolateral medulla were examined using in situ hybridization histochemistry for prolactin-releasing peptide mRNA .
	manualset3
116191	3	403652	13	NULL	NULL	0	NULL	nociceptive stimulus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , the effects of restraint stress , nociceptive stimulus and acute inflammatory stress on the expression of the prolactin-releasing peptide mRNA in the dorsomedial hypothalamic nucleus , nucleus of the solitary tract and ventrolateral medulla were examined using in situ hybridization histochemistry for prolactin-releasing peptide mRNA .
	manualset3
116192	4	403652	13	NULL	NULL	0	NULL	acute inflammatory stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , the effects of restraint stress , nociceptive stimulus and acute inflammatory stress on the expression of the prolactin-releasing peptide mRNA in the dorsomedial hypothalamic nucleus , nucleus of the solitary tract and ventrolateral medulla were examined using in situ hybridization histochemistry for prolactin-releasing peptide mRNA .
	manualset3
116193	5	403652	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , the effects of restraint stress , nociceptive stimulus and acute inflammatory stress on the expression of the prolactin-releasing peptide mRNA in the dorsomedial hypothalamic nucleus , nucleus of the solitary tract and ventrolateral medulla were examined using in situ hybridization histochemistry for prolactin-releasing peptide mRNA .
	manualset3
116194	6	403652	13	NULL	NULL	0	NULL	prolactin-releasing peptide mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , the effects of restraint stress , nociceptive stimulus and acute inflammatory stress on the expression of the prolactin-releasing peptide mRNA in the dorsomedial hypothalamic nucleus , nucleus of the solitary tract and ventrolateral medulla were examined using in situ hybridization histochemistry for prolactin-releasing peptide mRNA .
	manualset3
116195	7	403652	13	NULL	NULL	0	NULL	dorsomedial hypothalamic nucleus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , the effects of restraint stress , nociceptive stimulus and acute inflammatory stress on the expression of the prolactin-releasing peptide mRNA in the dorsomedial hypothalamic nucleus , nucleus of the solitary tract and ventrolateral medulla were examined using in situ hybridization histochemistry for prolactin-releasing peptide mRNA .
	manualset3
116196	8	403652	13	NULL	NULL	0	NULL	 nucleus of the solitary tract 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , the effects of restraint stress , nociceptive stimulus and acute inflammatory stress on the expression of the prolactin-releasing peptide mRNA in the dorsomedial hypothalamic nucleus , nucleus of the solitary tract and ventrolateral medulla were examined using in situ hybridization histochemistry for prolactin-releasing peptide mRNA .
	manualset3
116197	9	403652	13	NULL	NULL	0	NULL	ventrolateral medulla 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , the effects of restraint stress , nociceptive stimulus and acute inflammatory stress on the expression of the prolactin-releasing peptide mRNA in the dorsomedial hypothalamic nucleus , nucleus of the solitary tract and ventrolateral medulla were examined using in situ hybridization histochemistry for prolactin-releasing peptide mRNA .
	manualset3
116198	10	403652	13	NULL	NULL	0	NULL	in situ hybridization histochemistry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , the effects of restraint stress , nociceptive stimulus and acute inflammatory stress on the expression of the prolactin-releasing peptide mRNA in the dorsomedial hypothalamic nucleus , nucleus of the solitary tract and ventrolateral medulla were examined using in situ hybridization histochemistry for prolactin-releasing peptide mRNA .
	manualset3
116199	11	403652	13	NULL	NULL	0	NULL	prolactin-releasing peptide mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , the effects of restraint stress , nociceptive stimulus and acute inflammatory stress on the expression of the prolactin-releasing peptide mRNA in the dorsomedial hypothalamic nucleus , nucleus of the solitary tract and ventrolateral medulla were examined using in situ hybridization histochemistry for prolactin-releasing peptide mRNA .
	manualset3
116200	1	403653	13	NULL	NULL	0	NULL	localization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , the localization of pWEE1B was examined by immunohistochemistry , and exclusive nuclear localization was revealed in the fully grown oocytes .
	manualset3
116201	2	403653	13	NULL	NULL	0	NULL	pWEE1B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , the localization of pWEE1B was examined by immunohistochemistry , and exclusive nuclear localization was revealed in the fully grown oocytes .
	manualset3
116202	3	403653	13	NULL	NULL	0	NULL	 immunohistochemistry 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , the localization of pWEE1B was examined by immunohistochemistry , and exclusive nuclear localization was revealed in the fully grown oocytes .
	manualset3
116203	4	403653	13	NULL	NULL	0	NULL	exclusive nuclear localization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , the localization of pWEE1B was examined by immunohistochemistry , and exclusive nuclear localization was revealed in the fully grown oocytes .
	manualset3
116204	5	403653	13	NULL	NULL	0	NULL	 fully grown oocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , the localization of pWEE1B was examined by immunohistochemistry , and exclusive nuclear localization was revealed in the fully grown oocytes .
	manualset3
116205	1	403654	13	NULL	NULL	0	NULL	bias	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , they consider bias that occurs when the assumption that the latency period is a fixed constant does not hold .
	manualset3
116206	2	403654	13	NULL	NULL	0	NULL	assumption	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , they consider bias that occurs when the assumption that the latency period is a fixed constant does not hold .
	manualset3
116207	3	403654	13	NULL	NULL	0	NULL	latency period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , they consider bias that occurs when the assumption that the latency period is a fixed constant does not hold .
	manualset3
116208	4	403654	13	NULL	NULL	0	NULL	constant	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , they consider bias that occurs when the assumption that the latency period is a fixed constant does not hold .
	manualset3
116209	1	403655	13	NULL	NULL	0	NULL	density functional calculations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , using validated density functional calculations of a full chemical representation of FeMo-co and its connected residues ( alpha-275 ( Cys ) , alpha-442 ( His ) ) , I have characterized more than 80 possibilities for the coordination of up to three H atoms , and H ( 2 ) , and H + H ( 2 ) , on the S2A , Fe2 , S2B , Fe6 , S3B domain of FeMo-co , which is favored by recent targeted mutagenesis results .
	manualset3
116210	2	403655	13	NULL	NULL	0	NULL	full chemical representation	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , using validated density functional calculations of a full chemical representation of FeMo-co and its connected residues ( alpha-275 ( Cys ) , alpha-442 ( His ) ) , I have characterized more than 80 possibilities for the coordination of up to three H atoms , and H ( 2 ) , and H + H ( 2 ) , on the S2A , Fe2 , S2B , Fe6 , S3B domain of FeMo-co , which is favored by recent targeted mutagenesis results .
	manualset3
116211	3	403655	13	NULL	NULL	NULL	NULL	FeMo-co	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Next , using validated density functional calculations of a full chemical representation of FeMo-co and its connected residues ( alpha-275 ( Cys ) , alpha-442 ( His ) ) , I have characterized more than 80 possibilities for the coordination of up to three H atoms , and H ( 2 ) , and H + H ( 2 ) , on the S2A , Fe2 , S2B , Fe6 , S3B domain of FeMo-co , which is favored by recent targeted mutagenesis results .
	manualset3
116212	4	403655	13	NULL	NULL	0	NULL	residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , using validated density functional calculations of a full chemical representation of FeMo-co and its connected residues ( alpha-275 ( Cys ) , alpha-442 ( His ) ) , I have characterized more than 80 possibilities for the coordination of up to three H atoms , and H ( 2 ) , and H + H ( 2 ) , on the S2A , Fe2 , S2B , Fe6 , S3B domain of FeMo-co , which is favored by recent targeted mutagenesis results .
	manualset3
116213	5	403655	13	NULL	NULL	0	NULL	alpha-275 ( Cys ) 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , using validated density functional calculations of a full chemical representation of FeMo-co and its connected residues ( alpha-275 ( Cys ) , alpha-442 ( His ) ) , I have characterized more than 80 possibilities for the coordination of up to three H atoms , and H ( 2 ) , and H + H ( 2 ) , on the S2A , Fe2 , S2B , Fe6 , S3B domain of FeMo-co , which is favored by recent targeted mutagenesis results .
	manualset3
116214	6	403655	13	NULL	NULL	0	NULL	alpha-442 ( His ) 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , using validated density functional calculations of a full chemical representation of FeMo-co and its connected residues ( alpha-275 ( Cys ) , alpha-442 ( His ) ) , I have characterized more than 80 possibilities for the coordination of up to three H atoms , and H ( 2 ) , and H + H ( 2 ) , on the S2A , Fe2 , S2B , Fe6 , S3B domain of FeMo-co , which is favored by recent targeted mutagenesis results .
	manualset3
116215	7	403655	13	NULL	NULL	0	NULL	80 possibilities 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , using validated density functional calculations of a full chemical representation of FeMo-co and its connected residues ( alpha-275 ( Cys ) , alpha-442 ( His ) ) , I have characterized more than 80 possibilities for the coordination of up to three H atoms , and H ( 2 ) , and H + H ( 2 ) , on the S2A , Fe2 , S2B , Fe6 , S3B domain of FeMo-co , which is favored by recent targeted mutagenesis results .
	manualset3
116216	8	403655	13	NULL	NULL	0	NULL	coordination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , using validated density functional calculations of a full chemical representation of FeMo-co and its connected residues ( alpha-275 ( Cys ) , alpha-442 ( His ) ) , I have characterized more than 80 possibilities for the coordination of up to three H atoms , and H ( 2 ) , and H + H ( 2 ) , on the S2A , Fe2 , S2B , Fe6 , S3B domain of FeMo-co , which is favored by recent targeted mutagenesis results .
	manualset3
116217	9	403655	13	NULL	NULL	0	NULL	three H atoms	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , using validated density functional calculations of a full chemical representation of FeMo-co and its connected residues ( alpha-275 ( Cys ) , alpha-442 ( His ) ) , I have characterized more than 80 possibilities for the coordination of up to three H atoms , and H ( 2 ) , and H + H ( 2 ) , on the S2A , Fe2 , S2B , Fe6 , S3B domain of FeMo-co , which is favored by recent targeted mutagenesis results .
	manualset3
116218	10	403655	13	NULL	NULL	0	NULL	H ( 2 ) 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , using validated density functional calculations of a full chemical representation of FeMo-co and its connected residues ( alpha-275 ( Cys ) , alpha-442 ( His ) ) , I have characterized more than 80 possibilities for the coordination of up to three H atoms , and H ( 2 ) , and H + H ( 2 ) , on the S2A , Fe2 , S2B , Fe6 , S3B domain of FeMo-co , which is favored by recent targeted mutagenesis results .
	manualset3
116219	11	403655	13	NULL	NULL	0	NULL	H + H ( 2 )	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , using validated density functional calculations of a full chemical representation of FeMo-co and its connected residues ( alpha-275 ( Cys ) , alpha-442 ( His ) ) , I have characterized more than 80 possibilities for the coordination of up to three H atoms , and H ( 2 ) , and H + H ( 2 ) , on the S2A , Fe2 , S2B , Fe6 , S3B domain of FeMo-co , which is favored by recent targeted mutagenesis results .
	manualset3
116220	12	403655	13	NULL	NULL	0	NULL	S2A domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , using validated density functional calculations of a full chemical representation of FeMo-co and its connected residues ( alpha-275 ( Cys ) , alpha-442 ( His ) ) , I have characterized more than 80 possibilities for the coordination of up to three H atoms , and H ( 2 ) , and H + H ( 2 ) , on the S2A , Fe2 , S2B , Fe6 , S3B domain of FeMo-co , which is favored by recent targeted mutagenesis results .
	manualset3
116221	13	403655	13	NULL	NULL	0	NULL	Fe2 domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , using validated density functional calculations of a full chemical representation of FeMo-co and its connected residues ( alpha-275 ( Cys ) , alpha-442 ( His ) ) , I have characterized more than 80 possibilities for the coordination of up to three H atoms , and H ( 2 ) , and H + H ( 2 ) , on the S2A , Fe2 , S2B , Fe6 , S3B domain of FeMo-co , which is favored by recent targeted mutagenesis results .
	manualset3
116222	14	403655	13	NULL	NULL	0	NULL	S2B domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , using validated density functional calculations of a full chemical representation of FeMo-co and its connected residues ( alpha-275 ( Cys ) , alpha-442 ( His ) ) , I have characterized more than 80 possibilities for the coordination of up to three H atoms , and H ( 2 ) , and H + H ( 2 ) , on the S2A , Fe2 , S2B , Fe6 , S3B domain of FeMo-co , which is favored by recent targeted mutagenesis results .
	manualset3
116223	15	403655	13	NULL	NULL	0	NULL	Fe6 domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , using validated density functional calculations of a full chemical representation of FeMo-co and its connected residues ( alpha-275 ( Cys ) , alpha-442 ( His ) ) , I have characterized more than 80 possibilities for the coordination of up to three H atoms , and H ( 2 ) , and H + H ( 2 ) , on the S2A , Fe2 , S2B , Fe6 , S3B domain of FeMo-co , which is favored by recent targeted mutagenesis results .
	manualset3
116224	16	403655	13	NULL	NULL	0	NULL	S3B domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , using validated density functional calculations of a full chemical representation of FeMo-co and its connected residues ( alpha-275 ( Cys ) , alpha-442 ( His ) ) , I have characterized more than 80 possibilities for the coordination of up to three H atoms , and H ( 2 ) , and H + H ( 2 ) , on the S2A , Fe2 , S2B , Fe6 , S3B domain of FeMo-co , which is favored by recent targeted mutagenesis results .
	manualset3
116225	17	403655	13	NULL	NULL	0	NULL	FeMo-co	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , using validated density functional calculations of a full chemical representation of FeMo-co and its connected residues ( alpha-275 ( Cys ) , alpha-442 ( His ) ) , I have characterized more than 80 possibilities for the coordination of up to three H atoms , and H ( 2 ) , and H + H ( 2 ) , on the S2A , Fe2 , S2B , Fe6 , S3B domain of FeMo-co , which is favored by recent targeted mutagenesis results .
	manualset3
116226	18	403655	13	NULL	NULL	0	NULL	mutagenesis results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , using validated density functional calculations of a full chemical representation of FeMo-co and its connected residues ( alpha-275 ( Cys ) , alpha-442 ( His ) ) , I have characterized more than 80 possibilities for the coordination of up to three H atoms , and H ( 2 ) , and H + H ( 2 ) , on the S2A , Fe2 , S2B , Fe6 , S3B domain of FeMo-co , which is favored by recent targeted mutagenesis results .
	manualset3
116227	1	403656	13	NULL	NULL	0	NULL	Nicergoline	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Nicergoline enhances glutamate re-uptake and protects against brain damage in rat global brain ischemia .
	manualset3
116228	2	403656	13	NULL	NULL	0	NULL	glutamate re-uptake	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nicergoline enhances glutamate re-uptake and protects against brain damage in rat global brain ischemia .
	manualset3
116229	3	403656	13	NULL	NULL	0	NULL	brain damage 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nicergoline enhances glutamate re-uptake and protects against brain damage in rat global brain ischemia .
	manualset3
116230	4	403656	13	NULL	NULL	0	NULL	rat global brain ischemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nicergoline enhances glutamate re-uptake and protects against brain damage in rat global brain ischemia .
	manualset3
116231	1	403657	13	NULL	NULL	0	NULL	Nicotinamide 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Nicotinamide decreases nitric oxide production and partially protects human pancreatic islets against the suppressive effects of combinations of cytokines .
	manualset3
116232	2	403657	13	NULL	NULL	0	NULL	nitric oxide production 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nicotinamide decreases nitric oxide production and partially protects human pancreatic islets against the suppressive effects of combinations of cytokines .
	manualset3
116233	3	403657	13	NULL	NULL	0	NULL	human pancreatic islets	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Nicotinamide decreases nitric oxide production and partially protects human pancreatic islets against the suppressive effects of combinations of cytokines .
	manualset3
116234	4	403657	13	NULL	NULL	0	NULL	suppressive effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nicotinamide decreases nitric oxide production and partially protects human pancreatic islets against the suppressive effects of combinations of cytokines .
	manualset3
116235	5	403657	13	NULL	NULL	0	NULL	combinations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nicotinamide decreases nitric oxide production and partially protects human pancreatic islets against the suppressive effects of combinations of cytokines .
	manualset3
116236	6	403657	13	NULL	NULL	0	NULL	cytokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nicotinamide decreases nitric oxide production and partially protects human pancreatic islets against the suppressive effects of combinations of cytokines .
	manualset3
116237	1	403658	13	NULL	NULL	0	NULL	Nicotine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Nicotine 's opioid and anti-opioid interactions : proposed role in smoking behavior .
	manualset3
116238	2	403658	13	NULL	NULL	NULL	NULL	opioid interactions	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nicotine 's opioid and anti-opioid interactions : proposed role in smoking behavior .
	manualset3
116239	3	403658	13	NULL	NULL	NULL	NULL	anti-opioid interactions	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nicotine 's opioid and anti-opioid interactions : proposed role in smoking behavior .
	manualset3
116240	4	403658	13	NULL	NULL	0	NULL	role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nicotine 's opioid and anti-opioid interactions : proposed role in smoking behavior .
	manualset3
116241	5	403658	13	NULL	NULL	0	NULL	smoking behavior	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nicotine 's opioid and anti-opioid interactions : proposed role in smoking behavior .
	manualset3
116242	1	403659	13	NULL	NULL	0	NULL	Nine-week-old rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine-week-old rats were instrumented to record aortic BP in the conscious state .
	manualset3
116243	2	403659	13	NULL	NULL	0	NULL	aortic BP 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine-week-old rats were instrumented to record aortic BP in the conscious state .
	manualset3
116244	3	403659	13	NULL	NULL	0	NULL	conscious state	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine-week-old rats were instrumented to record aortic BP in the conscious state .
	manualset3
116245	1	403660	13	NULL	NULL	0	NULL	Nine adenovirus strains 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine adenovirus strains isolated from chimpanzees were studied with regard to their relatedness to each other and to human adenovirus prototypes by neutralization and hemagglutination inhibition .
	manualset3
116246	2	403660	13	NULL	NULL	0	NULL	chimpanzees	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine adenovirus strains isolated from chimpanzees were studied with regard to their relatedness to each other and to human adenovirus prototypes by neutralization and hemagglutination inhibition .
	manualset3
116247	3	403660	13	NULL	NULL	0	NULL	regard	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine adenovirus strains isolated from chimpanzees were studied with regard to their relatedness to each other and to human adenovirus prototypes by neutralization and hemagglutination inhibition .
	manualset3
116248	4	403660	13	NULL	NULL	0	NULL	relatedness	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine adenovirus strains isolated from chimpanzees were studied with regard to their relatedness to each other and to human adenovirus prototypes by neutralization and hemagglutination inhibition .
	manualset3
116249	5	403660	13	NULL	NULL	0	NULL	 human adenovirus prototypes 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine adenovirus strains isolated from chimpanzees were studied with regard to their relatedness to each other and to human adenovirus prototypes by neutralization and hemagglutination inhibition .
	manualset3
116250	6	403660	13	NULL	NULL	NULL	NULL	neutralization	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nine adenovirus strains isolated from chimpanzees were studied with regard to their relatedness to each other and to human adenovirus prototypes by neutralization and hemagglutination inhibition .
	manualset3
116251	7	403660	13	NULL	NULL	NULL	NULL	hemagglutination inhibition	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nine adenovirus strains isolated from chimpanzees were studied with regard to their relatedness to each other and to human adenovirus prototypes by neutralization and hemagglutination inhibition .
	manualset3
116252	1	403661	13	NULL	NULL	0	NULL	Nine cases	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine cases of aberrations involving chromosome 18 are used to illustrate the use and clinical potential of array CGH .
	manualset3
116253	2	403661	13	NULL	NULL	0	NULL	aberrations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine cases of aberrations involving chromosome 18 are used to illustrate the use and clinical potential of array CGH .
	manualset3
116254	3	403661	13	NULL	NULL	0	NULL	chromosome 18 	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine cases of aberrations involving chromosome 18 are used to illustrate the use and clinical potential of array CGH .
	manualset3
116255	4	403661	13	NULL	NULL	0	NULL	use	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine cases of aberrations involving chromosome 18 are used to illustrate the use and clinical potential of array CGH .
	manualset3
116256	5	403661	13	NULL	NULL	0	NULL	clinical potential	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine cases of aberrations involving chromosome 18 are used to illustrate the use and clinical potential of array CGH .
	manualset3
116257	6	403661	13	NULL	NULL	0	NULL	array CGH 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine cases of aberrations involving chromosome 18 are used to illustrate the use and clinical potential of array CGH .
	manualset3
116258	1	403662	13	NULL	NULL	0	NULL	Nine moss species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine moss species showed antibacterial activity against Gram ( + ) bacteria , in particular H. splendens and its ethyl acetate fractions showed stronger activity .
	manualset3
116259	2	403662	13	NULL	NULL	0	NULL	antibacterial activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine moss species showed antibacterial activity against Gram ( + ) bacteria , in particular H. splendens and its ethyl acetate fractions showed stronger activity .
	manualset3
116260	3	403662	13	NULL	NULL	0	NULL	Gram ( + ) bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine moss species showed antibacterial activity against Gram ( + ) bacteria , in particular H. splendens and its ethyl acetate fractions showed stronger activity .
	manualset3
116261	4	403662	13	NULL	NULL	0	NULL	 H. splendens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine moss species showed antibacterial activity against Gram ( + ) bacteria , in particular H. splendens and its ethyl acetate fractions showed stronger activity .
	manualset3
116262	5	403662	13	NULL	NULL	0	NULL	ethyl acetate fractions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine moss species showed antibacterial activity against Gram ( + ) bacteria , in particular H. splendens and its ethyl acetate fractions showed stronger activity .
	manualset3
116263	6	403662	13	NULL	NULL	0	NULL	stronger activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine moss species showed antibacterial activity against Gram ( + ) bacteria , in particular H. splendens and its ethyl acetate fractions showed stronger activity .
	manualset3
116264	1	403663	13	NULL	NULL	0	NULL	Nine patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine patients suffering from hypothyroidism due to thyroid ectopia or hypogenesis , with a large sella turcica , were examined at adolescence or during adult life .
	manualset3
116265	2	403663	13	NULL	NULL	0	NULL	suffering 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine patients suffering from hypothyroidism due to thyroid ectopia or hypogenesis , with a large sella turcica , were examined at adolescence or during adult life .
	manualset3
116266	3	403663	13	NULL	NULL	0	NULL	hypothyroidism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine patients suffering from hypothyroidism due to thyroid ectopia or hypogenesis , with a large sella turcica , were examined at adolescence or during adult life .
	manualset3
116267	4	403663	13	NULL	NULL	0	NULL	thyroid ectopia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine patients suffering from hypothyroidism due to thyroid ectopia or hypogenesis , with a large sella turcica , were examined at adolescence or during adult life .
	manualset3
116268	5	403663	13	NULL	NULL	0	NULL	hypogenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine patients suffering from hypothyroidism due to thyroid ectopia or hypogenesis , with a large sella turcica , were examined at adolescence or during adult life .
	manualset3
116269	6	403663	13	NULL	NULL	0	NULL	sella turcica	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine patients suffering from hypothyroidism due to thyroid ectopia or hypogenesis , with a large sella turcica , were examined at adolescence or during adult life .
	manualset3
116270	7	403663	13	NULL	NULL	0	NULL	adolescence	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine patients suffering from hypothyroidism due to thyroid ectopia or hypogenesis , with a large sella turcica , were examined at adolescence or during adult life .
	manualset3
116271	8	403663	13	NULL	NULL	0	NULL	adult life 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine patients suffering from hypothyroidism due to thyroid ectopia or hypogenesis , with a large sella turcica , were examined at adolescence or during adult life .
	manualset3
116272	1	403664	13	NULL	NULL	0	NULL	Nine patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine patients with neither Delirium Tremens nor seizure , needing a lumbar puncture for their medical problem , were matched by sex and by age .
	manualset3
116273	2	403664	13	NULL	NULL	0	NULL	Delirium Tremens	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine patients with neither Delirium Tremens nor seizure , needing a lumbar puncture for their medical problem , were matched by sex and by age .
	manualset3
116274	3	403664	13	NULL	NULL	0	NULL	seizure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine patients with neither Delirium Tremens nor seizure , needing a lumbar puncture for their medical problem , were matched by sex and by age .
	manualset3
116275	4	403664	13	NULL	NULL	0	NULL	lumbar puncture	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine patients with neither Delirium Tremens nor seizure , needing a lumbar puncture for their medical problem , were matched by sex and by age .
	manualset3
116276	5	403664	13	NULL	NULL	0	NULL	medical problem 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine patients with neither Delirium Tremens nor seizure , needing a lumbar puncture for their medical problem , were matched by sex and by age .
	manualset3
116277	6	403664	13	NULL	NULL	0	NULL	sex 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine patients with neither Delirium Tremens nor seizure , needing a lumbar puncture for their medical problem , were matched by sex and by age .
	manualset3
116278	7	403664	13	NULL	NULL	0	NULL	age 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine patients with neither Delirium Tremens nor seizure , needing a lumbar puncture for their medical problem , were matched by sex and by age .
	manualset3
116279	1	403665	13	NULL	NULL	0	NULL	Nine subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine subjects with acquired ATIII deficiency also received ATIII treatment for venous or arterial thrombosis or disseminated intravascular coagulation , all with low plasma ATIII levels .
	manualset3
116280	2	403665	13	NULL	NULL	0	NULL	acquired ATIII deficiency 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine subjects with acquired ATIII deficiency also received ATIII treatment for venous or arterial thrombosis or disseminated intravascular coagulation , all with low plasma ATIII levels .
	manualset3
116281	3	403665	13	NULL	NULL	0	NULL	ATIII treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine subjects with acquired ATIII deficiency also received ATIII treatment for venous or arterial thrombosis or disseminated intravascular coagulation , all with low plasma ATIII levels .
	manualset3
116282	4	403665	13	NULL	NULL	0	NULL	venous thrombosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine subjects with acquired ATIII deficiency also received ATIII treatment for venous or arterial thrombosis or disseminated intravascular coagulation , all with low plasma ATIII levels .
	manualset3
116283	5	403665	13	NULL	NULL	0	NULL	arterial thrombosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine subjects with acquired ATIII deficiency also received ATIII treatment for venous or arterial thrombosis or disseminated intravascular coagulation , all with low plasma ATIII levels .
	manualset3
116284	6	403665	13	NULL	NULL	0	NULL	disseminated intravascular coagulation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine subjects with acquired ATIII deficiency also received ATIII treatment for venous or arterial thrombosis or disseminated intravascular coagulation , all with low plasma ATIII levels .
	manualset3
116285	7	403665	13	NULL	NULL	0	NULL	low plasma ATIII levels 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nine subjects with acquired ATIII deficiency also received ATIII treatment for venous or arterial thrombosis or disseminated intravascular coagulation , all with low plasma ATIII levels .
	manualset3
116286	1	403666	13	NULL	NULL	0	NULL	Nineteen patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nineteen patients with upper motor neuron paralysis received 57 HVOBS and 114 PEGBS trials in a crossover design .
	manualset3
116287	2	403666	13	NULL	NULL	0	NULL	upper motor neuron paralysis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nineteen patients with upper motor neuron paralysis received 57 HVOBS and 114 PEGBS trials in a crossover design .
	manualset3
116288	3	403666	13	NULL	NULL	0	NULL	57 HVOBS trials	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Nineteen patients with upper motor neuron paralysis received 57 HVOBS and 114 PEGBS trials in a crossover design .
	manualset3
116289	4	403666	13	NULL	NULL	0	NULL	114 PEGBS trials 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Nineteen patients with upper motor neuron paralysis received 57 HVOBS and 114 PEGBS trials in a crossover design .
	manualset3
116290	5	403666	13	NULL	NULL	0	NULL	crossover design 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Nineteen patients with upper motor neuron paralysis received 57 HVOBS and 114 PEGBS trials in a crossover design .
	manualset3
116291	1	403667	13	NULL	NULL	0	NULL	Biological characteristics	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Biological characteristics of the invasive stage of Myxosoma cerebralis ( Myxosporidia : Myxosomatidae ) ) .
	manualset3
116292	2	403667	13	NULL	NULL	0	NULL	invasive stage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Biological characteristics of the invasive stage of Myxosoma cerebralis ( Myxosporidia : Myxosomatidae ) ) .
	manualset3
116293	3	403667	13	NULL	NULL	0	NULL	Myxosoma cerebralis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Biological characteristics of the invasive stage of Myxosoma cerebralis ( Myxosporidia : Myxosomatidae ) ) .
	manualset3
116294	4	403667	13	NULL	NULL	0	NULL	Myxosporidia	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Biological characteristics of the invasive stage of Myxosoma cerebralis ( Myxosporidia : Myxosomatidae ) ) .
	manualset3
116295	5	403667	13	NULL	NULL	0	NULL	Myxosomatidae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Biological characteristics of the invasive stage of Myxosoma cerebralis ( Myxosporidia : Myxosomatidae ) ) .
	manualset3
116296	1	403668	13	NULL	NULL	0	NULL	inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A complete inhibition of E-selectin and ICAM-1 expression was observed when antibodies against TNF-alpha and IL-1 beta were added to plasma prior to the incubation to endothelial cultures .
	manualset3
116297	2	403668	13	NULL	NULL	0	NULL	E-selectin expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A complete inhibition of E-selectin and ICAM-1 expression was observed when antibodies against TNF-alpha and IL-1 beta were added to plasma prior to the incubation to endothelial cultures .
	manualset3
116298	3	403668	13	NULL	NULL	0	NULL	ICAM-1 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A complete inhibition of E-selectin and ICAM-1 expression was observed when antibodies against TNF-alpha and IL-1 beta were added to plasma prior to the incubation to endothelial cultures .
	manualset3
116299	4	403668	13	NULL	NULL	0	NULL	antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A complete inhibition of E-selectin and ICAM-1 expression was observed when antibodies against TNF-alpha and IL-1 beta were added to plasma prior to the incubation to endothelial cultures .
	manualset3
116300	5	403668	13	NULL	NULL	0	NULL	TNF-alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A complete inhibition of E-selectin and ICAM-1 expression was observed when antibodies against TNF-alpha and IL-1 beta were added to plasma prior to the incubation to endothelial cultures .
	manualset3
116301	6	403668	13	NULL	NULL	0	NULL	IL-1 beta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A complete inhibition of E-selectin and ICAM-1 expression was observed when antibodies against TNF-alpha and IL-1 beta were added to plasma prior to the incubation to endothelial cultures .
	manualset3
116302	7	403668	13	NULL	NULL	0	NULL	plasma	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A complete inhibition of E-selectin and ICAM-1 expression was observed when antibodies against TNF-alpha and IL-1 beta were added to plasma prior to the incubation to endothelial cultures .
	manualset3
116303	8	403668	13	NULL	NULL	0	NULL	incubation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A complete inhibition of E-selectin and ICAM-1 expression was observed when antibodies against TNF-alpha and IL-1 beta were added to plasma prior to the incubation to endothelial cultures .
	manualset3
116304	9	403668	13	NULL	NULL	0	NULL	endothelial cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A complete inhibition of E-selectin and ICAM-1 expression was observed when antibodies against TNF-alpha and IL-1 beta were added to plasma prior to the incubation to endothelial cultures .
	manualset3
116305	1	403669	13	NULL	NULL	0	NULL	Ninety-four patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-four patients with bipolar disorder participating in a random-assignment , double-blind , prospective maintenance trial of standard - ( 0.8 to 1.0 mmol/L ) vs low-range ( 0.4 to 0.6 mmol/L ) serum lithium levels were assessed to determine the presence and significance of subsyndromal symptoms during periods of remission and recovery .
	manualset3
116306	2	403669	13	NULL	NULL	0	NULL	bipolar disorder	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-four patients with bipolar disorder participating in a random-assignment , double-blind , prospective maintenance trial of standard - ( 0.8 to 1.0 mmol/L ) vs low-range ( 0.4 to 0.6 mmol/L ) serum lithium levels were assessed to determine the presence and significance of subsyndromal symptoms during periods of remission and recovery .
	manualset3
116307	3	403669	13	NULL	NULL	0	NULL	random-assignment , double-blind , prospective maintenance trial 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-four patients with bipolar disorder participating in a random-assignment , double-blind , prospective maintenance trial of standard - ( 0.8 to 1.0 mmol/L ) vs low-range ( 0.4 to 0.6 mmol/L ) serum lithium levels were assessed to determine the presence and significance of subsyndromal symptoms during periods of remission and recovery .
	manualset3
116308	4	403669	13	NULL	NULL	0	NULL	 standard - ( 0.8 to 1.0 mmol/L ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-four patients with bipolar disorder participating in a random-assignment , double-blind , prospective maintenance trial of standard - ( 0.8 to 1.0 mmol/L ) vs low-range ( 0.4 to 0.6 mmol/L ) serum lithium levels were assessed to determine the presence and significance of subsyndromal symptoms during periods of remission and recovery .
	manualset3
116309	5	403669	13	NULL	NULL	0	NULL	low-range ( 0.4 to 0.6 mmol/L )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-four patients with bipolar disorder participating in a random-assignment , double-blind , prospective maintenance trial of standard - ( 0.8 to 1.0 mmol/L ) vs low-range ( 0.4 to 0.6 mmol/L ) serum lithium levels were assessed to determine the presence and significance of subsyndromal symptoms during periods of remission and recovery .
	manualset3
116310	6	403669	13	NULL	NULL	0	NULL	serum lithium levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-four patients with bipolar disorder participating in a random-assignment , double-blind , prospective maintenance trial of standard - ( 0.8 to 1.0 mmol/L ) vs low-range ( 0.4 to 0.6 mmol/L ) serum lithium levels were assessed to determine the presence and significance of subsyndromal symptoms during periods of remission and recovery .
	manualset3
116311	7	403669	13	NULL	NULL	0	NULL	presence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-four patients with bipolar disorder participating in a random-assignment , double-blind , prospective maintenance trial of standard - ( 0.8 to 1.0 mmol/L ) vs low-range ( 0.4 to 0.6 mmol/L ) serum lithium levels were assessed to determine the presence and significance of subsyndromal symptoms during periods of remission and recovery .
	manualset3
116312	8	403669	13	NULL	NULL	0	NULL	significance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-four patients with bipolar disorder participating in a random-assignment , double-blind , prospective maintenance trial of standard - ( 0.8 to 1.0 mmol/L ) vs low-range ( 0.4 to 0.6 mmol/L ) serum lithium levels were assessed to determine the presence and significance of subsyndromal symptoms during periods of remission and recovery .
	manualset3
116313	9	403669	13	NULL	NULL	0	NULL	subsyndromal symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-four patients with bipolar disorder participating in a random-assignment , double-blind , prospective maintenance trial of standard - ( 0.8 to 1.0 mmol/L ) vs low-range ( 0.4 to 0.6 mmol/L ) serum lithium levels were assessed to determine the presence and significance of subsyndromal symptoms during periods of remission and recovery .
	manualset3
116314	10	403669	13	NULL	NULL	0	NULL	periods of remission	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-four patients with bipolar disorder participating in a random-assignment , double-blind , prospective maintenance trial of standard - ( 0.8 to 1.0 mmol/L ) vs low-range ( 0.4 to 0.6 mmol/L ) serum lithium levels were assessed to determine the presence and significance of subsyndromal symptoms during periods of remission and recovery .
	manualset3
116315	11	403669	13	NULL	NULL	0	NULL	 periods of recovery	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-four patients with bipolar disorder participating in a random-assignment , double-blind , prospective maintenance trial of standard - ( 0.8 to 1.0 mmol/L ) vs low-range ( 0.4 to 0.6 mmol/L ) serum lithium levels were assessed to determine the presence and significance of subsyndromal symptoms during periods of remission and recovery .
	manualset3
116316	1	403670	13	NULL	NULL	0	NULL	Ninety-one percent 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-one percent of the strains isolated in the final study period were observed to have MIC levels ) or = 0.125 mg/L to ciprofloxacin .
	manualset3
116317	2	403670	13	NULL	NULL	0	NULL	strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-one percent of the strains isolated in the final study period were observed to have MIC levels ) or = 0.125 mg/L to ciprofloxacin .
	manualset3
116318	3	403670	13	NULL	NULL	0	NULL	final study period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-one percent of the strains isolated in the final study period were observed to have MIC levels ) or = 0.125 mg/L to ciprofloxacin .
	manualset3
116319	4	403670	13	NULL	NULL	0	NULL	MIC levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-one percent of the strains isolated in the final study period were observed to have MIC levels ) or = 0.125 mg/L to ciprofloxacin .
	manualset3
116320	5	403670	13	NULL	NULL	0	NULL	0.125 mg/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-one percent of the strains isolated in the final study period were observed to have MIC levels ) or = 0.125 mg/L to ciprofloxacin .
	manualset3
116321	6	403670	13	NULL	NULL	0	NULL	ciprofloxacin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-one percent of the strains isolated in the final study period were observed to have MIC levels ) or = 0.125 mg/L to ciprofloxacin .
	manualset3
116322	1	403671	13	NULL	NULL	0	NULL	Ninety-six women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-six women of advanced maternal age were interviewed about the way they obtained information on prenatal diagnosis and about how the decision was made as to what procedure was to be performed ( transabdominal chorionic villus sampling ( TA-CVS ) or amniocentesis ) .
	manualset3
116323	2	403671	13	NULL	NULL	0	NULL	maternal age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-six women of advanced maternal age were interviewed about the way they obtained information on prenatal diagnosis and about how the decision was made as to what procedure was to be performed ( transabdominal chorionic villus sampling ( TA-CVS ) or amniocentesis ) .
	manualset3
116324	3	403671	13	NULL	NULL	0	NULL	way	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-six women of advanced maternal age were interviewed about the way they obtained information on prenatal diagnosis and about how the decision was made as to what procedure was to be performed ( transabdominal chorionic villus sampling ( TA-CVS ) or amniocentesis ) .
	manualset3
116325	4	403671	13	NULL	NULL	0	NULL	information	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-six women of advanced maternal age were interviewed about the way they obtained information on prenatal diagnosis and about how the decision was made as to what procedure was to be performed ( transabdominal chorionic villus sampling ( TA-CVS ) or amniocentesis ) .
	manualset3
116326	5	403671	13	NULL	NULL	0	NULL	prenatal diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-six women of advanced maternal age were interviewed about the way they obtained information on prenatal diagnosis and about how the decision was made as to what procedure was to be performed ( transabdominal chorionic villus sampling ( TA-CVS ) or amniocentesis ) .
	manualset3
116327	6	403671	13	NULL	NULL	0	NULL	decision	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-six women of advanced maternal age were interviewed about the way they obtained information on prenatal diagnosis and about how the decision was made as to what procedure was to be performed ( transabdominal chorionic villus sampling ( TA-CVS ) or amniocentesis ) .
	manualset3
116328	7	403671	13	NULL	NULL	0	NULL	procedure 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-six women of advanced maternal age were interviewed about the way they obtained information on prenatal diagnosis and about how the decision was made as to what procedure was to be performed ( transabdominal chorionic villus sampling ( TA-CVS ) or amniocentesis ) .
	manualset3
116329	8	403671	13	NULL	NULL	0	NULL	transabdominal chorionic villus sampling ( TA-CVS ) 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-six women of advanced maternal age were interviewed about the way they obtained information on prenatal diagnosis and about how the decision was made as to what procedure was to be performed ( transabdominal chorionic villus sampling ( TA-CVS ) or amniocentesis ) .
	manualset3
116330	9	403671	13	NULL	NULL	0	NULL	amniocentesis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-six women of advanced maternal age were interviewed about the way they obtained information on prenatal diagnosis and about how the decision was made as to what procedure was to be performed ( transabdominal chorionic villus sampling ( TA-CVS ) or amniocentesis ) .
	manualset3
116331	1	403672	13	NULL	NULL	0	NULL	Ninety-three ( 93 ) patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-three ( 93 ) patients ( 58.5 % ) had symptoms of a sleep disturbance .
	manualset3
116332	2	403672	13	NULL	NULL	0	NULL	58.5 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-three ( 93 ) patients ( 58.5 % ) had symptoms of a sleep disturbance .
	manualset3
116333	3	403672	13	NULL	NULL	0	NULL	symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-three ( 93 ) patients ( 58.5 % ) had symptoms of a sleep disturbance .
	manualset3
116334	4	403672	13	NULL	NULL	0	NULL	sleep disturbance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-three ( 93 ) patients ( 58.5 % ) had symptoms of a sleep disturbance .
	manualset3
116335	1	403673	13	NULL	NULL	0	NULL	Ninety-three percent	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-three percent of control patients compared to 25 % of PED/CPS patients were satisfied with surgery ( P & lt ; 0.001 ) .
	manualset3
116336	2	403673	13	NULL	NULL	0	NULL	control patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-three percent of control patients compared to 25 % of PED/CPS patients were satisfied with surgery ( P & lt ; 0.001 ) .
	manualset3
116337	3	403673	13	NULL	NULL	0	NULL	25 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-three percent of control patients compared to 25 % of PED/CPS patients were satisfied with surgery ( P & lt ; 0.001 ) .
	manualset3
116338	4	403673	13	NULL	NULL	0	NULL	PED/CPS patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-three percent of control patients compared to 25 % of PED/CPS patients were satisfied with surgery ( P & lt ; 0.001 ) .
	manualset3
116339	5	403673	13	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-three percent of control patients compared to 25 % of PED/CPS patients were satisfied with surgery ( P & lt ; 0.001 ) .
	manualset3
116340	6	403673	13	NULL	NULL	0	NULL	P & lt ; 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety-three percent of control patients compared to 25 % of PED/CPS patients were satisfied with surgery ( P & lt ; 0.001 ) .
	manualset3
116341	1	403674	13	NULL	NULL	0	NULL	Ninety crude extracts 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety crude extracts , including dichloromethane , methanol and aqueous extracts from 30 medicinal plants used in the Yemeni ethnomedicine to treat common infections , were screened in vitro for antimicrobial activities against three Gram-positive bacteria and two Gram-negative bacteria , Candida maltosa and five opportunistic human fungal pathogens ( two yeasts , three hyphomycetes ) .
	manualset3
116342	2	403674	13	NULL	NULL	0	NULL	dichloromethane	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety crude extracts , including dichloromethane , methanol and aqueous extracts from 30 medicinal plants used in the Yemeni ethnomedicine to treat common infections , were screened in vitro for antimicrobial activities against three Gram-positive bacteria and two Gram-negative bacteria , Candida maltosa and five opportunistic human fungal pathogens ( two yeasts , three hyphomycetes ) .
	manualset3
116343	3	403674	13	NULL	NULL	0	NULL	methanol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety crude extracts , including dichloromethane , methanol and aqueous extracts from 30 medicinal plants used in the Yemeni ethnomedicine to treat common infections , were screened in vitro for antimicrobial activities against three Gram-positive bacteria and two Gram-negative bacteria , Candida maltosa and five opportunistic human fungal pathogens ( two yeasts , three hyphomycetes ) .
	manualset3
116344	4	403674	13	NULL	NULL	0	NULL	aqueous extracts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety crude extracts , including dichloromethane , methanol and aqueous extracts from 30 medicinal plants used in the Yemeni ethnomedicine to treat common infections , were screened in vitro for antimicrobial activities against three Gram-positive bacteria and two Gram-negative bacteria , Candida maltosa and five opportunistic human fungal pathogens ( two yeasts , three hyphomycetes ) .
	manualset3
116345	5	403674	13	NULL	NULL	0	NULL	30 medicinal plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety crude extracts , including dichloromethane , methanol and aqueous extracts from 30 medicinal plants used in the Yemeni ethnomedicine to treat common infections , were screened in vitro for antimicrobial activities against three Gram-positive bacteria and two Gram-negative bacteria , Candida maltosa and five opportunistic human fungal pathogens ( two yeasts , three hyphomycetes ) .
	manualset3
116346	6	403674	13	NULL	NULL	0	NULL	Yemeni ethnomedicine	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety crude extracts , including dichloromethane , methanol and aqueous extracts from 30 medicinal plants used in the Yemeni ethnomedicine to treat common infections , were screened in vitro for antimicrobial activities against three Gram-positive bacteria and two Gram-negative bacteria , Candida maltosa and five opportunistic human fungal pathogens ( two yeasts , three hyphomycetes ) .
	manualset3
116347	7	403674	13	NULL	NULL	0	NULL	common infections 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety crude extracts , including dichloromethane , methanol and aqueous extracts from 30 medicinal plants used in the Yemeni ethnomedicine to treat common infections , were screened in vitro for antimicrobial activities against three Gram-positive bacteria and two Gram-negative bacteria , Candida maltosa and five opportunistic human fungal pathogens ( two yeasts , three hyphomycetes ) .
	manualset3
116348	8	403674	13	NULL	NULL	0	NULL	antimicrobial activities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety crude extracts , including dichloromethane , methanol and aqueous extracts from 30 medicinal plants used in the Yemeni ethnomedicine to treat common infections , were screened in vitro for antimicrobial activities against three Gram-positive bacteria and two Gram-negative bacteria , Candida maltosa and five opportunistic human fungal pathogens ( two yeasts , three hyphomycetes ) .
	manualset3
116349	9	403674	13	NULL	NULL	0	NULL	three Gram-positive bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety crude extracts , including dichloromethane , methanol and aqueous extracts from 30 medicinal plants used in the Yemeni ethnomedicine to treat common infections , were screened in vitro for antimicrobial activities against three Gram-positive bacteria and two Gram-negative bacteria , Candida maltosa and five opportunistic human fungal pathogens ( two yeasts , three hyphomycetes ) .
	manualset3
116350	10	403674	13	NULL	NULL	0	NULL	two Gram-negative bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety crude extracts , including dichloromethane , methanol and aqueous extracts from 30 medicinal plants used in the Yemeni ethnomedicine to treat common infections , were screened in vitro for antimicrobial activities against three Gram-positive bacteria and two Gram-negative bacteria , Candida maltosa and five opportunistic human fungal pathogens ( two yeasts , three hyphomycetes ) .
	manualset3
116351	11	403674	13	NULL	NULL	0	NULL	Candida maltosa	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety crude extracts , including dichloromethane , methanol and aqueous extracts from 30 medicinal plants used in the Yemeni ethnomedicine to treat common infections , were screened in vitro for antimicrobial activities against three Gram-positive bacteria and two Gram-negative bacteria , Candida maltosa and five opportunistic human fungal pathogens ( two yeasts , three hyphomycetes ) .
	manualset3
116352	12	403674	13	NULL	NULL	0	NULL	five opportunistic human fungal pathogens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety crude extracts , including dichloromethane , methanol and aqueous extracts from 30 medicinal plants used in the Yemeni ethnomedicine to treat common infections , were screened in vitro for antimicrobial activities against three Gram-positive bacteria and two Gram-negative bacteria , Candida maltosa and five opportunistic human fungal pathogens ( two yeasts , three hyphomycetes ) .
	manualset3
116353	13	403674	13	NULL	NULL	0	NULL	 two yeasts	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety crude extracts , including dichloromethane , methanol and aqueous extracts from 30 medicinal plants used in the Yemeni ethnomedicine to treat common infections , were screened in vitro for antimicrobial activities against three Gram-positive bacteria and two Gram-negative bacteria , Candida maltosa and five opportunistic human fungal pathogens ( two yeasts , three hyphomycetes ) .
	manualset3
116354	14	403674	13	NULL	NULL	0	NULL	three hyphomycetes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety crude extracts , including dichloromethane , methanol and aqueous extracts from 30 medicinal plants used in the Yemeni ethnomedicine to treat common infections , were screened in vitro for antimicrobial activities against three Gram-positive bacteria and two Gram-negative bacteria , Candida maltosa and five opportunistic human fungal pathogens ( two yeasts , three hyphomycetes ) .
	manualset3
116355	1	403675	13	NULL	NULL	0	NULL	Ninety percent	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety percent ( 18 of 20 ) of the tumors induced in male F344 rats harbored mutations , which were detected in three of four adenomas ( 75 % ) and 15 of 16 adenocarcinomas ( 94 % ) .
	manualset3
116356	2	403675	13	NULL	NULL	0	NULL	18 of 20 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety percent ( 18 of 20 ) of the tumors induced in male F344 rats harbored mutations , which were detected in three of four adenomas ( 75 % ) and 15 of 16 adenocarcinomas ( 94 % ) .
	manualset3
116357	3	403675	13	NULL	NULL	0	NULL	tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety percent ( 18 of 20 ) of the tumors induced in male F344 rats harbored mutations , which were detected in three of four adenomas ( 75 % ) and 15 of 16 adenocarcinomas ( 94 % ) .
	manualset3
116358	4	403675	13	NULL	NULL	0	NULL	male F344 rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety percent ( 18 of 20 ) of the tumors induced in male F344 rats harbored mutations , which were detected in three of four adenomas ( 75 % ) and 15 of 16 adenocarcinomas ( 94 % ) .
	manualset3
116359	5	403675	13	NULL	NULL	0	NULL	mutations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety percent ( 18 of 20 ) of the tumors induced in male F344 rats harbored mutations , which were detected in three of four adenomas ( 75 % ) and 15 of 16 adenocarcinomas ( 94 % ) .
	manualset3
116360	6	403675	13	NULL	NULL	0	NULL	three of four adenomas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety percent ( 18 of 20 ) of the tumors induced in male F344 rats harbored mutations , which were detected in three of four adenomas ( 75 % ) and 15 of 16 adenocarcinomas ( 94 % ) .
	manualset3
116361	7	403675	13	NULL	NULL	0	NULL	75 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety percent ( 18 of 20 ) of the tumors induced in male F344 rats harbored mutations , which were detected in three of four adenomas ( 75 % ) and 15 of 16 adenocarcinomas ( 94 % ) .
	manualset3
116362	8	403675	13	NULL	NULL	0	NULL	15 of 16 adenocarcinomas 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety percent ( 18 of 20 ) of the tumors induced in male F344 rats harbored mutations , which were detected in three of four adenomas ( 75 % ) and 15 of 16 adenocarcinomas ( 94 % ) .
	manualset3
116363	9	403675	13	NULL	NULL	0	NULL	94 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ninety percent ( 18 of 20 ) of the tumors induced in male F344 rats harbored mutations , which were detected in three of four adenomas ( 75 % ) and 15 of 16 adenocarcinomas ( 94 % ) .
	manualset3
116364	1	403676	13	NULL	NULL	0	NULL	 loss 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A complete loss of Brg1 expression was observed in 5 ( 8.3 % ) of the 60 lesions .
	manualset3
116365	2	403676	13	NULL	NULL	0	NULL	Brg1 expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A complete loss of Brg1 expression was observed in 5 ( 8.3 % ) of the 60 lesions .
	manualset3
116366	3	403676	13	NULL	NULL	0	NULL	 5 ( 8.3 % ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A complete loss of Brg1 expression was observed in 5 ( 8.3 % ) of the 60 lesions .
	manualset3
116367	4	403676	13	NULL	NULL	0	NULL	60 lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A complete loss of Brg1 expression was observed in 5 ( 8.3 % ) of the 60 lesions .
	manualset3
116368	1	403677	13	NULL	NULL	0	NULL	Nipple discharge	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nipple discharge is a common condition , and the diagnosis and treatment is discussed .
	manualset3
116369	2	403677	13	NULL	NULL	0	NULL	common condition 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nipple discharge is a common condition , and the diagnosis and treatment is discussed .
	manualset3
116370	3	403677	13	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Nipple discharge is a common condition , and the diagnosis and treatment is discussed .
	manualset3
116371	4	403677	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Nipple discharge is a common condition , and the diagnosis and treatment is discussed .
	manualset3
116372	1	403678	13	NULL	NULL	0	NULL	NitR 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	NitR was found to be a regulator of S. meliloti hmgA expression under nitrogen deprivation conditions , suggesting the presence of a ntr-independent nitrogen deprivation regulatory system .
	manualset3
116373	2	403678	13	NULL	NULL	0	NULL	regulator	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	NitR was found to be a regulator of S. meliloti hmgA expression under nitrogen deprivation conditions , suggesting the presence of a ntr-independent nitrogen deprivation regulatory system .
	manualset3
116374	3	403678	13	NULL	NULL	0	NULL	S. meliloti hmgA expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	NitR was found to be a regulator of S. meliloti hmgA expression under nitrogen deprivation conditions , suggesting the presence of a ntr-independent nitrogen deprivation regulatory system .
	manualset3
116375	4	403678	13	NULL	NULL	0	NULL	nitrogen deprivation conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	NitR was found to be a regulator of S. meliloti hmgA expression under nitrogen deprivation conditions , suggesting the presence of a ntr-independent nitrogen deprivation regulatory system .
	manualset3
116376	5	403678	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	NitR was found to be a regulator of S. meliloti hmgA expression under nitrogen deprivation conditions , suggesting the presence of a ntr-independent nitrogen deprivation regulatory system .
	manualset3
116377	6	403678	13	NULL	NULL	0	NULL	nitrogen deprivation regulatory system	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	NitR was found to be a regulator of S. meliloti hmgA expression under nitrogen deprivation conditions , suggesting the presence of a ntr-independent nitrogen deprivation regulatory system .
	manualset3
116378	1	403679	13	NULL	NULL	0	NULL	Nitric oxide ( NO ) production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide ( NO ) production , as detectable by indirect and direct methods , as well as the expression of inducible nitric oxide synthase ( iNOS ) in the intestinal mucosa appear to be enhanced in active ulcerative colitis and , when in excess , to play a proinflammatory role in the disease .
	manualset3
116379	2	403679	13	NULL	NULL	0	NULL	methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide ( NO ) production , as detectable by indirect and direct methods , as well as the expression of inducible nitric oxide synthase ( iNOS ) in the intestinal mucosa appear to be enhanced in active ulcerative colitis and , when in excess , to play a proinflammatory role in the disease .
	manualset3
116380	3	403679	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide ( NO ) production , as detectable by indirect and direct methods , as well as the expression of inducible nitric oxide synthase ( iNOS ) in the intestinal mucosa appear to be enhanced in active ulcerative colitis and , when in excess , to play a proinflammatory role in the disease .
	manualset3
116381	4	403679	13	NULL	NULL	0	NULL	inducible nitric oxide synthase ( iNOS ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide ( NO ) production , as detectable by indirect and direct methods , as well as the expression of inducible nitric oxide synthase ( iNOS ) in the intestinal mucosa appear to be enhanced in active ulcerative colitis and , when in excess , to play a proinflammatory role in the disease .
	manualset3
116382	5	403679	13	NULL	NULL	0	NULL	intestinal mucosa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide ( NO ) production , as detectable by indirect and direct methods , as well as the expression of inducible nitric oxide synthase ( iNOS ) in the intestinal mucosa appear to be enhanced in active ulcerative colitis and , when in excess , to play a proinflammatory role in the disease .
	manualset3
116383	6	403679	13	NULL	NULL	0	NULL	ulcerative colitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide ( NO ) production , as detectable by indirect and direct methods , as well as the expression of inducible nitric oxide synthase ( iNOS ) in the intestinal mucosa appear to be enhanced in active ulcerative colitis and , when in excess , to play a proinflammatory role in the disease .
	manualset3
116384	7	403679	13	NULL	NULL	0	NULL	proinflammatory role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide ( NO ) production , as detectable by indirect and direct methods , as well as the expression of inducible nitric oxide synthase ( iNOS ) in the intestinal mucosa appear to be enhanced in active ulcerative colitis and , when in excess , to play a proinflammatory role in the disease .
	manualset3
116385	8	403679	13	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide ( NO ) production , as detectable by indirect and direct methods , as well as the expression of inducible nitric oxide synthase ( iNOS ) in the intestinal mucosa appear to be enhanced in active ulcerative colitis and , when in excess , to play a proinflammatory role in the disease .
	manualset3
116386	9	403679	13	NULL	NULL	0	NULL	excess 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide ( NO ) production , as detectable by indirect and direct methods , as well as the expression of inducible nitric oxide synthase ( iNOS ) in the intestinal mucosa appear to be enhanced in active ulcerative colitis and , when in excess , to play a proinflammatory role in the disease .
	manualset3
116387	1	403680	13	NULL	NULL	0	NULL	Nitric oxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide : a predictor of morbidity in postoperative patients ?
	manualset3
116388	2	403680	13	NULL	NULL	0	NULL	predictor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide : a predictor of morbidity in postoperative patients ?
	manualset3
116389	3	403680	13	NULL	NULL	0	NULL	morbidity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide : a predictor of morbidity in postoperative patients ?
	manualset3
116390	4	403680	13	NULL	NULL	0	NULL	postoperative patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide : a predictor of morbidity in postoperative patients ?
	manualset3
116391	1	403681	13	NULL	NULL	0	NULL	Nitric oxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide in plant immunity .
	manualset3
116392	2	403681	13	NULL	NULL	0	NULL	plant immunity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide in plant immunity .
	manualset3
116393	1	403682	13	NULL	NULL	0	NULL	Nitric oxide 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide produced exogenously by the addition of NO donors was able to delay or inhibit apoptosis induced by a combination of tumor necrosis factor alpha and actinomycin D and to suppress the activity of caspase 3 .
	manualset3
116394	2	403682	13	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide produced exogenously by the addition of NO donors was able to delay or inhibit apoptosis induced by a combination of tumor necrosis factor alpha and actinomycin D and to suppress the activity of caspase 3 .
	manualset3
116395	3	403682	13	NULL	NULL	0	NULL	NO donors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide produced exogenously by the addition of NO donors was able to delay or inhibit apoptosis induced by a combination of tumor necrosis factor alpha and actinomycin D and to suppress the activity of caspase 3 .
	manualset3
116396	4	403682	13	NULL	NULL	0	NULL	apoptosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide produced exogenously by the addition of NO donors was able to delay or inhibit apoptosis induced by a combination of tumor necrosis factor alpha and actinomycin D and to suppress the activity of caspase 3 .
	manualset3
116397	5	403682	13	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide produced exogenously by the addition of NO donors was able to delay or inhibit apoptosis induced by a combination of tumor necrosis factor alpha and actinomycin D and to suppress the activity of caspase 3 .
	manualset3
116398	6	403682	13	NULL	NULL	0	NULL	tumor necrosis factor alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide produced exogenously by the addition of NO donors was able to delay or inhibit apoptosis induced by a combination of tumor necrosis factor alpha and actinomycin D and to suppress the activity of caspase 3 .
	manualset3
116399	7	403682	13	NULL	NULL	0	NULL	actinomycin D 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide produced exogenously by the addition of NO donors was able to delay or inhibit apoptosis induced by a combination of tumor necrosis factor alpha and actinomycin D and to suppress the activity of caspase 3 .
	manualset3
116400	8	403682	13	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide produced exogenously by the addition of NO donors was able to delay or inhibit apoptosis induced by a combination of tumor necrosis factor alpha and actinomycin D and to suppress the activity of caspase 3 .
	manualset3
116401	9	403682	13	NULL	NULL	0	NULL	caspase 3 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide produced exogenously by the addition of NO donors was able to delay or inhibit apoptosis induced by a combination of tumor necrosis factor alpha and actinomycin D and to suppress the activity of caspase 3 .
	manualset3
116402	1	403683	13	NULL	NULL	0	NULL	Nitric oxide release	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide release accounts for the reduced incidence of cutaneous infections in psoriasis .
	manualset3
116403	2	403683	13	NULL	NULL	0	NULL	incidence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide release accounts for the reduced incidence of cutaneous infections in psoriasis .
	manualset3
116404	3	403683	13	NULL	NULL	0	NULL	cutaneous infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide release accounts for the reduced incidence of cutaneous infections in psoriasis .
	manualset3
116405	4	403683	13	NULL	NULL	0	NULL	psoriasis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide release accounts for the reduced incidence of cutaneous infections in psoriasis .
	manualset3
116406	1	403684	13	NULL	NULL	0	NULL	Nitric oxide synthase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide synthase inhibition by pentacycloundecane conjugates of aminoguanidine and tryptamine .
	manualset3
116407	2	403684	13	NULL	NULL	0	NULL	inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide synthase inhibition by pentacycloundecane conjugates of aminoguanidine and tryptamine .
	manualset3
116408	3	403684	13	NULL	NULL	0	NULL	pentacycloundecane conjugates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide synthase inhibition by pentacycloundecane conjugates of aminoguanidine and tryptamine .
	manualset3
116409	4	403684	13	NULL	NULL	0	NULL	aminoguanidine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide synthase inhibition by pentacycloundecane conjugates of aminoguanidine and tryptamine .
	manualset3
116410	5	403684	13	NULL	NULL	0	NULL	tryptamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide synthase inhibition by pentacycloundecane conjugates of aminoguanidine and tryptamine .
	manualset3
116411	1	403685	13	NULL	NULL	0	NULL	Nitroglycerin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitroglycerin given with tissue-type plasminogen activator ( t-PA ) has been shown to decrease the thrombolytic effect of t-PA in animal models of coronary artery thrombosis .
	manualset3
116412	2	403685	13	NULL	NULL	0	NULL	tissue-type plasminogen activator ( t-PA )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitroglycerin given with tissue-type plasminogen activator ( t-PA ) has been shown to decrease the thrombolytic effect of t-PA in animal models of coronary artery thrombosis .
	manualset3
116413	3	403685	13	NULL	NULL	0	NULL	thrombolytic effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitroglycerin given with tissue-type plasminogen activator ( t-PA ) has been shown to decrease the thrombolytic effect of t-PA in animal models of coronary artery thrombosis .
	manualset3
116414	4	403685	13	NULL	NULL	0	NULL	 t-PA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitroglycerin given with tissue-type plasminogen activator ( t-PA ) has been shown to decrease the thrombolytic effect of t-PA in animal models of coronary artery thrombosis .
	manualset3
116415	5	403685	13	NULL	NULL	0	NULL	 animal models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitroglycerin given with tissue-type plasminogen activator ( t-PA ) has been shown to decrease the thrombolytic effect of t-PA in animal models of coronary artery thrombosis .
	manualset3
116416	6	403685	13	NULL	NULL	0	NULL	coronary artery thrombosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitroglycerin given with tissue-type plasminogen activator ( t-PA ) has been shown to decrease the thrombolytic effect of t-PA in animal models of coronary artery thrombosis .
	manualset3
116417	1	403686	13	NULL	NULL	0	NULL	Nitromethane ( NM )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitromethane ( NM ) , dimethylnitramine ( DMNA ) , and isopropylnitrate ( IPN ) are used as model molecules for C-NO ( 2 ) , N-NO ( 2 ) , and O-NO ( 2 ) active moieties , respectively .
	manualset3
116418	2	403686	13	NULL	NULL	0	NULL	dimethylnitramine ( DMNA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitromethane ( NM ) , dimethylnitramine ( DMNA ) , and isopropylnitrate ( IPN ) are used as model molecules for C-NO ( 2 ) , N-NO ( 2 ) , and O-NO ( 2 ) active moieties , respectively .
	manualset3
116419	3	403686	13	NULL	NULL	0	NULL	isopropylnitrate ( IPN ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitromethane ( NM ) , dimethylnitramine ( DMNA ) , and isopropylnitrate ( IPN ) are used as model molecules for C-NO ( 2 ) , N-NO ( 2 ) , and O-NO ( 2 ) active moieties , respectively .
	manualset3
116420	4	403686	13	NULL	NULL	0	NULL	model molecules 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitromethane ( NM ) , dimethylnitramine ( DMNA ) , and isopropylnitrate ( IPN ) are used as model molecules for C-NO ( 2 ) , N-NO ( 2 ) , and O-NO ( 2 ) active moieties , respectively .
	manualset3
116421	5	403686	13	NULL	NULL	NULL	NULL	C-NO ( 2 ) active moieties	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nitromethane ( NM ) , dimethylnitramine ( DMNA ) , and isopropylnitrate ( IPN ) are used as model molecules for C-NO ( 2 ) , N-NO ( 2 ) , and O-NO ( 2 ) active moieties , respectively .
	manualset3
116422	6	403686	13	NULL	NULL	NULL	NULL	N-NO ( 2 ) active moieties	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nitromethane ( NM ) , dimethylnitramine ( DMNA ) , and isopropylnitrate ( IPN ) are used as model molecules for C-NO ( 2 ) , N-NO ( 2 ) , and O-NO ( 2 ) active moieties , respectively .
	manualset3
116423	7	403686	13	NULL	NULL	0	NULL	O-NO ( 2 ) active moieties	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitromethane ( NM ) , dimethylnitramine ( DMNA ) , and isopropylnitrate ( IPN ) are used as model molecules for C-NO ( 2 ) , N-NO ( 2 ) , and O-NO ( 2 ) active moieties , respectively .
	manualset3
116424	1	403687	13	NULL	NULL	0	NULL	Nitromethane	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitromethane was identified as a particularly suitable photolytic precursor of methyl for studies by photoionization and threshold photoelectron spectroscopy .
	manualset3
116425	2	403687	13	NULL	NULL	0	NULL	photolytic precursor 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitromethane was identified as a particularly suitable photolytic precursor of methyl for studies by photoionization and threshold photoelectron spectroscopy .
	manualset3
116426	3	403687	13	NULL	NULL	0	NULL	methyl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitromethane was identified as a particularly suitable photolytic precursor of methyl for studies by photoionization and threshold photoelectron spectroscopy .
	manualset3
116427	4	403687	13	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitromethane was identified as a particularly suitable photolytic precursor of methyl for studies by photoionization and threshold photoelectron spectroscopy .
	manualset3
116428	5	403687	13	NULL	NULL	0	NULL	photoionization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitromethane was identified as a particularly suitable photolytic precursor of methyl for studies by photoionization and threshold photoelectron spectroscopy .
	manualset3
116429	6	403687	13	NULL	NULL	0	NULL	threshold photoelectron spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitromethane was identified as a particularly suitable photolytic precursor of methyl for studies by photoionization and threshold photoelectron spectroscopy .
	manualset3
116430	1	403688	13	NULL	NULL	0	NULL	Nm23 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nm23 was found to be expressed in all the tissue specimens .
	manualset3
116431	2	403688	13	NULL	NULL	0	NULL	tissue specimens 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Nm23 was found to be expressed in all the tissue specimens .
	manualset3
116432	1	403689	13	NULL	NULL	0	NULL	Gs protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	No Gs protein could be detected in the CT1-producing cultures .
	manualset3
116433	2	403689	13	NULL	NULL	0	NULL	CT1-producing cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	No Gs protein could be detected in the CT1-producing cultures .
	manualset3
116434	1	403690	13	NULL	NULL	0	NULL	Y. enterocolitica 4/O : 3	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	No Y. enterocolitica 4/O : 3 was isolated from meat strips of hind leg .
	manualset3
116435	2	403690	13	NULL	NULL	0	NULL	meat strips	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	No Y. enterocolitica 4/O : 3 was isolated from meat strips of hind leg .
	manualset3
116436	3	403690	13	NULL	NULL	0	NULL	hind leg	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	No Y. enterocolitica 4/O : 3 was isolated from meat strips of hind leg .
	manualset3
116437	1	403691	13	NULL	NULL	0	NULL	abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No abnormalities were found in calcium ion uptake by the sarcoplasmic reticulum .
	manualset3
116438	2	403691	13	NULL	NULL	0	NULL	calcium ion uptake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	No abnormalities were found in calcium ion uptake by the sarcoplasmic reticulum .
	manualset3
116439	3	403691	13	NULL	NULL	0	NULL	sarcoplasmic reticulum	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	No abnormalities were found in calcium ion uptake by the sarcoplasmic reticulum .
	manualset3
116457	1	403692	13	NULL	NULL	0	NULL	additivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No additivity of hybridization values could be detected when RNAs from two different tissues were mixed , which suggests that BALB/c mouse liver , kidney , uterus and embryo transcribe a common set of nucleic acid sequences of the homologous regions of the N - and X-tropic viral genomes , in addition to other sequences of the same region that are specific for indiviual tissues .
	manualset3
116458	2	403692	13	NULL	NULL	0	NULL	hybridization values 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No additivity of hybridization values could be detected when RNAs from two different tissues were mixed , which suggests that BALB/c mouse liver , kidney , uterus and embryo transcribe a common set of nucleic acid sequences of the homologous regions of the N - and X-tropic viral genomes , in addition to other sequences of the same region that are specific for indiviual tissues .
	manualset3
116459	3	403692	13	NULL	NULL	0	NULL	RNAs 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	No additivity of hybridization values could be detected when RNAs from two different tissues were mixed , which suggests that BALB/c mouse liver , kidney , uterus and embryo transcribe a common set of nucleic acid sequences of the homologous regions of the N - and X-tropic viral genomes , in addition to other sequences of the same region that are specific for indiviual tissues .
	manualset3
116460	4	403692	13	NULL	NULL	0	NULL	two different tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	No additivity of hybridization values could be detected when RNAs from two different tissues were mixed , which suggests that BALB/c mouse liver , kidney , uterus and embryo transcribe a common set of nucleic acid sequences of the homologous regions of the N - and X-tropic viral genomes , in addition to other sequences of the same region that are specific for indiviual tissues .
	manualset3
116461	5	403692	13	NULL	NULL	0	NULL	BALB/c mouse	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	No additivity of hybridization values could be detected when RNAs from two different tissues were mixed , which suggests that BALB/c mouse liver , kidney , uterus and embryo transcribe a common set of nucleic acid sequences of the homologous regions of the N - and X-tropic viral genomes , in addition to other sequences of the same region that are specific for indiviual tissues .
	manualset3
116462	6	403692	13	NULL	NULL	0	NULL	liver 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	No additivity of hybridization values could be detected when RNAs from two different tissues were mixed , which suggests that BALB/c mouse liver , kidney , uterus and embryo transcribe a common set of nucleic acid sequences of the homologous regions of the N - and X-tropic viral genomes , in addition to other sequences of the same region that are specific for indiviual tissues .
	manualset3
116463	7	403692	13	NULL	NULL	0	NULL	kidney	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	No additivity of hybridization values could be detected when RNAs from two different tissues were mixed , which suggests that BALB/c mouse liver , kidney , uterus and embryo transcribe a common set of nucleic acid sequences of the homologous regions of the N - and X-tropic viral genomes , in addition to other sequences of the same region that are specific for indiviual tissues .
	manualset3
116464	8	403692	13	NULL	NULL	0	NULL	uterus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	No additivity of hybridization values could be detected when RNAs from two different tissues were mixed , which suggests that BALB/c mouse liver , kidney , uterus and embryo transcribe a common set of nucleic acid sequences of the homologous regions of the N - and X-tropic viral genomes , in addition to other sequences of the same region that are specific for indiviual tissues .
	manualset3
116465	9	403692	13	NULL	NULL	0	NULL	embryo 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	No additivity of hybridization values could be detected when RNAs from two different tissues were mixed , which suggests that BALB/c mouse liver , kidney , uterus and embryo transcribe a common set of nucleic acid sequences of the homologous regions of the N - and X-tropic viral genomes , in addition to other sequences of the same region that are specific for indiviual tissues .
	manualset3
116466	10	403692	13	NULL	NULL	0	NULL	common set	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	No additivity of hybridization values could be detected when RNAs from two different tissues were mixed , which suggests that BALB/c mouse liver , kidney , uterus and embryo transcribe a common set of nucleic acid sequences of the homologous regions of the N - and X-tropic viral genomes , in addition to other sequences of the same region that are specific for indiviual tissues .
	manualset3
116467	11	403692	13	NULL	NULL	0	NULL	nucleic acid sequences 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	No additivity of hybridization values could be detected when RNAs from two different tissues were mixed , which suggests that BALB/c mouse liver , kidney , uterus and embryo transcribe a common set of nucleic acid sequences of the homologous regions of the N - and X-tropic viral genomes , in addition to other sequences of the same region that are specific for indiviual tissues .
	manualset3
116468	12	403692	13	NULL	NULL	0	NULL	homologous regions	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	No additivity of hybridization values could be detected when RNAs from two different tissues were mixed , which suggests that BALB/c mouse liver , kidney , uterus and embryo transcribe a common set of nucleic acid sequences of the homologous regions of the N - and X-tropic viral genomes , in addition to other sequences of the same region that are specific for indiviual tissues .
	manualset3
116469	13	403692	13	NULL	NULL	0	NULL	N -tropic viral genomes 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	No additivity of hybridization values could be detected when RNAs from two different tissues were mixed , which suggests that BALB/c mouse liver , kidney , uterus and embryo transcribe a common set of nucleic acid sequences of the homologous regions of the N - and X-tropic viral genomes , in addition to other sequences of the same region that are specific for indiviual tissues .
	manualset3
116470	14	403692	13	NULL	NULL	0	NULL	X-tropic viral genomes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	No additivity of hybridization values could be detected when RNAs from two different tissues were mixed , which suggests that BALB/c mouse liver , kidney , uterus and embryo transcribe a common set of nucleic acid sequences of the homologous regions of the N - and X-tropic viral genomes , in addition to other sequences of the same region that are specific for indiviual tissues .
	manualset3
116471	15	403692	13	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No additivity of hybridization values could be detected when RNAs from two different tissues were mixed , which suggests that BALB/c mouse liver , kidney , uterus and embryo transcribe a common set of nucleic acid sequences of the homologous regions of the N - and X-tropic viral genomes , in addition to other sequences of the same region that are specific for indiviual tissues .
	manualset3
116472	16	403692	13	NULL	NULL	0	NULL	sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	No additivity of hybridization values could be detected when RNAs from two different tissues were mixed , which suggests that BALB/c mouse liver , kidney , uterus and embryo transcribe a common set of nucleic acid sequences of the homologous regions of the N - and X-tropic viral genomes , in addition to other sequences of the same region that are specific for indiviual tissues .
	manualset3
116473	17	403692	13	NULL	NULL	0	NULL	region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	No additivity of hybridization values could be detected when RNAs from two different tissues were mixed , which suggests that BALB/c mouse liver , kidney , uterus and embryo transcribe a common set of nucleic acid sequences of the homologous regions of the N - and X-tropic viral genomes , in addition to other sequences of the same region that are specific for indiviual tissues .
	manualset3
116474	18	403692	13	NULL	NULL	0	NULL	indiviual tissues 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	No additivity of hybridization values could be detected when RNAs from two different tissues were mixed , which suggests that BALB/c mouse liver , kidney , uterus and embryo transcribe a common set of nucleic acid sequences of the homologous regions of the N - and X-tropic viral genomes , in addition to other sequences of the same region that are specific for indiviual tissues .
	manualset3
116450	1	403693	13	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	No association was found between IL-6 levels and knee extensor muscle ( r = 0.087 , P = 0.306 ) or flexor ( r = -0.011 , P = 0.894 ) strength .
	manualset3
116451	2	403693	13	NULL	NULL	0	NULL	IL-6 levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	No association was found between IL-6 levels and knee extensor muscle ( r = 0.087 , P = 0.306 ) or flexor ( r = -0.011 , P = 0.894 ) strength .
	manualset3
116452	3	403693	13	NULL	NULL	0	NULL	knee extensor muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	No association was found between IL-6 levels and knee extensor muscle ( r = 0.087 , P = 0.306 ) or flexor ( r = -0.011 , P = 0.894 ) strength .
	manualset3
116453	4	403693	13	NULL	NULL	0	NULL	 r = 0.087 , P = 0.306	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No association was found between IL-6 levels and knee extensor muscle ( r = 0.087 , P = 0.306 ) or flexor ( r = -0.011 , P = 0.894 ) strength .
	manualset3
116454	5	403693	13	NULL	NULL	0	NULL	flexor	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	No association was found between IL-6 levels and knee extensor muscle ( r = 0.087 , P = 0.306 ) or flexor ( r = -0.011 , P = 0.894 ) strength .
	manualset3
116455	6	403693	13	NULL	NULL	0	NULL	r = -0.011 , P = 0.894	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No association was found between IL-6 levels and knee extensor muscle ( r = 0.087 , P = 0.306 ) or flexor ( r = -0.011 , P = 0.894 ) strength .
	manualset3
116456	7	403693	13	NULL	NULL	0	NULL	strength 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No association was found between IL-6 levels and knee extensor muscle ( r = 0.087 , P = 0.306 ) or flexor ( r = -0.011 , P = 0.894 ) strength .
	manualset3
116445	1	403694	13	NULL	NULL	0	NULL	cellular deformation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	No cellular deformation was observed following 2 micrograms-dose ; whereas 6 micrograms-dose caused significant damage of gametogenic cells .
	manualset3
116446	2	403694	13	NULL	NULL	0	NULL	2 micrograms-dose	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No cellular deformation was observed following 2 micrograms-dose ; whereas 6 micrograms-dose caused significant damage of gametogenic cells .
	manualset3
116447	3	403694	13	NULL	NULL	0	NULL	6 micrograms-dose	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No cellular deformation was observed following 2 micrograms-dose ; whereas 6 micrograms-dose caused significant damage of gametogenic cells .
	manualset3
116448	4	403694	13	NULL	NULL	0	NULL	damage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	No cellular deformation was observed following 2 micrograms-dose ; whereas 6 micrograms-dose caused significant damage of gametogenic cells .
	manualset3
116449	5	403694	13	NULL	NULL	0	NULL	gametogenic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	No cellular deformation was observed following 2 micrograms-dose ; whereas 6 micrograms-dose caused significant damage of gametogenic cells .
	manualset3
116440	1	403695	13	NULL	NULL	0	NULL	changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No changes were recorded for plasma calcitriol concentrations in response to P depletion with an adequate Ca supply .
	manualset3
116441	2	403695	13	NULL	NULL	0	NULL	plasma calcitriol concentrations 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No changes were recorded for plasma calcitriol concentrations in response to P depletion with an adequate Ca supply .
	manualset3
116442	3	403695	13	NULL	NULL	0	NULL	response	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No changes were recorded for plasma calcitriol concentrations in response to P depletion with an adequate Ca supply .
	manualset3
116443	4	403695	13	NULL	NULL	0	NULL	P depletion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No changes were recorded for plasma calcitriol concentrations in response to P depletion with an adequate Ca supply .
	manualset3
116444	5	403695	13	NULL	NULL	0	NULL	Ca 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	No changes were recorded for plasma calcitriol concentrations in response to P depletion with an adequate Ca supply .
	manualset3
116804	1	403696	13	NULL	NULL	0	NULL	complex linkage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A complex linkage between the cytoskeleton and the extracellular matrix is illustrated both in the cord forming Sertoli and granulosa cells , and in the adjacent mesenchymal cells .
	manualset3
116805	2	403696	13	NULL	NULL	0	NULL	cytoskeleton	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A complex linkage between the cytoskeleton and the extracellular matrix is illustrated both in the cord forming Sertoli and granulosa cells , and in the adjacent mesenchymal cells .
	manualset3
116806	3	403696	13	NULL	NULL	0	NULL	extracellular matrix	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A complex linkage between the cytoskeleton and the extracellular matrix is illustrated both in the cord forming Sertoli and granulosa cells , and in the adjacent mesenchymal cells .
	manualset3
116807	4	403696	13	NULL	NULL	0	NULL	cord forming Sertoli cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A complex linkage between the cytoskeleton and the extracellular matrix is illustrated both in the cord forming Sertoli and granulosa cells , and in the adjacent mesenchymal cells .
	manualset3
116808	5	403696	13	NULL	NULL	0	NULL	granulosa cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A complex linkage between the cytoskeleton and the extracellular matrix is illustrated both in the cord forming Sertoli and granulosa cells , and in the adjacent mesenchymal cells .
	manualset3
116809	6	403696	13	NULL	NULL	0	NULL	mesenchymal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A complex linkage between the cytoskeleton and the extracellular matrix is illustrated both in the cord forming Sertoli and granulosa cells , and in the adjacent mesenchymal cells .
	manualset3
116810	1	403697	13	NULL	NULL	0	NULL	correlations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	No close correlations between the anti-LPS and anti-Ipa antibody responses were observed indicating that they may be differently regulated .
	manualset3
116811	2	403697	13	NULL	NULL	0	NULL	anti-LPS antibody responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	No close correlations between the anti-LPS and anti-Ipa antibody responses were observed indicating that they may be differently regulated .
	manualset3
116812	3	403697	13	NULL	NULL	0	NULL	anti-Ipa antibody responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	No close correlations between the anti-LPS and anti-Ipa antibody responses were observed indicating that they may be differently regulated .
	manualset3
116813	1	403698	13	NULL	NULL	0	NULL	complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No complications related to the anastomosis , by Viz leakage , dehiscence , biliary stasis , or stenosis were observed .
	manualset3
116814	2	403698	13	NULL	NULL	0	NULL	anastomosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No complications related to the anastomosis , by Viz leakage , dehiscence , biliary stasis , or stenosis were observed .
	manualset3
116815	3	403698	13	NULL	NULL	0	NULL	Viz leakage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No complications related to the anastomosis , by Viz leakage , dehiscence , biliary stasis , or stenosis were observed .
	manualset3
116816	4	403698	13	NULL	NULL	0	NULL	dehiscence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No complications related to the anastomosis , by Viz leakage , dehiscence , biliary stasis , or stenosis were observed .
	manualset3
116817	5	403698	13	NULL	NULL	0	NULL	biliary stasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No complications related to the anastomosis , by Viz leakage , dehiscence , biliary stasis , or stenosis were observed .
	manualset3
116818	6	403698	13	NULL	NULL	0	NULL	stenosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No complications related to the anastomosis , by Viz leakage , dehiscence , biliary stasis , or stenosis were observed .
	manualset3
116820	1	403699	13	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	No correlation was found between ADL and the laterality of the lesion in both groups .
	manualset3
116821	2	403699	13	NULL	NULL	0	NULL	ADL	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No correlation was found between ADL and the laterality of the lesion in both groups .
	manualset3
116822	3	403699	13	NULL	NULL	0	NULL	laterality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No correlation was found between ADL and the laterality of the lesion in both groups .
	manualset3
116823	4	403699	13	NULL	NULL	0	NULL	lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No correlation was found between ADL and the laterality of the lesion in both groups .
	manualset3
116824	5	403699	13	NULL	NULL	0	NULL	groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No correlation was found between ADL and the laterality of the lesion in both groups .
	manualset3
116825	1	403700	13	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	No correlation was found between decrease in deformability and duration of the extracorporeal circulation procedure .
	manualset3
116826	2	403700	13	NULL	NULL	0	NULL	decrease 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No correlation was found between decrease in deformability and duration of the extracorporeal circulation procedure .
	manualset3
116827	3	403700	13	NULL	NULL	0	NULL	deformability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No correlation was found between decrease in deformability and duration of the extracorporeal circulation procedure .
	manualset3
116828	4	403700	13	NULL	NULL	0	NULL	duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	No correlation was found between decrease in deformability and duration of the extracorporeal circulation procedure .
	manualset3
116829	5	403700	13	NULL	NULL	0	NULL	extracorporeal circulation procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	No correlation was found between decrease in deformability and duration of the extracorporeal circulation procedure .
	manualset3
116830	1	403701	13	NULL	NULL	0	NULL	correlations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	No correlations were found between the reflex parameters and the degree of spasticity .
	manualset3
116831	2	403701	13	NULL	NULL	0	NULL	reflex parameters	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No correlations were found between the reflex parameters and the degree of spasticity .
	manualset3
116832	3	403701	13	NULL	NULL	0	NULL	degree of spasticity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No correlations were found between the reflex parameters and the degree of spasticity .
	manualset3
116833	1	403702	13	NULL	NULL	0	NULL	cross-reactivity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No cross-reactivity between the probes and the DNAs of mammalian cells , yeasts , or bacteria was noted .
	manualset3
116834	2	403702	13	NULL	NULL	0	NULL	probes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	No cross-reactivity between the probes and the DNAs of mammalian cells , yeasts , or bacteria was noted .
	manualset3
116835	3	403702	13	NULL	NULL	0	NULL	DNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	No cross-reactivity between the probes and the DNAs of mammalian cells , yeasts , or bacteria was noted .
	manualset3
116836	4	403702	13	NULL	NULL	0	NULL	mammalian cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	No cross-reactivity between the probes and the DNAs of mammalian cells , yeasts , or bacteria was noted .
	manualset3
116837	5	403702	13	NULL	NULL	0	NULL	yeasts	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	No cross-reactivity between the probes and the DNAs of mammalian cells , yeasts , or bacteria was noted .
	manualset3
116838	6	403702	13	NULL	NULL	0	NULL	bacteria 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	No cross-reactivity between the probes and the DNAs of mammalian cells , yeasts , or bacteria was noted .
	manualset3
116839	1	403703	13	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	No data exist regarding the effects of altitude exposure on sleep in children .
	manualset3
116840	2	403703	13	NULL	NULL	0	NULL	effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No data exist regarding the effects of altitude exposure on sleep in children .
	manualset3
116841	3	403703	13	NULL	NULL	0	NULL	altitude exposure	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	No data exist regarding the effects of altitude exposure on sleep in children .
	manualset3
116842	4	403703	13	NULL	NULL	0	NULL	sleep 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No data exist regarding the effects of altitude exposure on sleep in children .
	manualset3
116843	5	403703	13	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No data exist regarding the effects of altitude exposure on sleep in children .
	manualset3
116844	1	403704	13	NULL	NULL	0	NULL	difference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference could be detected either in fluid volume , nor in content or type of glycosaminoglycan , in the amnion of the two groups .
	manualset3
116845	2	403704	13	NULL	NULL	0	NULL	fluid volume	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference could be detected either in fluid volume , nor in content or type of glycosaminoglycan , in the amnion of the two groups .
	manualset3
116846	3	403704	13	NULL	NULL	0	NULL	content	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference could be detected either in fluid volume , nor in content or type of glycosaminoglycan , in the amnion of the two groups .
	manualset3
116847	4	403704	13	NULL	NULL	0	NULL	type of glycosaminoglycan	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference could be detected either in fluid volume , nor in content or type of glycosaminoglycan , in the amnion of the two groups .
	manualset3
116848	5	403704	13	NULL	NULL	0	NULL	amnion	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference could be detected either in fluid volume , nor in content or type of glycosaminoglycan , in the amnion of the two groups .
	manualset3
116849	6	403704	13	NULL	NULL	0	NULL	two groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference could be detected either in fluid volume , nor in content or type of glycosaminoglycan , in the amnion of the two groups .
	manualset3
116850	1	403705	13	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference from normal controls was observed with peripheral blood lymphocytes from either RA or SLE .
	manualset3
116851	2	403705	13	NULL	NULL	0	NULL	normal controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference from normal controls was observed with peripheral blood lymphocytes from either RA or SLE .
	manualset3
116852	3	403705	13	NULL	NULL	0	NULL	peripheral blood lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference from normal controls was observed with peripheral blood lymphocytes from either RA or SLE .
	manualset3
116853	4	403705	13	NULL	NULL	0	NULL	RA	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference from normal controls was observed with peripheral blood lymphocytes from either RA or SLE .
	manualset3
116854	5	403705	13	NULL	NULL	0	NULL	SLE	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference from normal controls was observed with peripheral blood lymphocytes from either RA or SLE .
	manualset3
117217	1	403706	13	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference in QoL was found between patients with PPMS and those with secondary progressive MS. The Italian FAMS questionnaire is a valid measure to assess the QoL concerns of patients with MS. FAMS is also easy to administer and is well accepted by patients .
	manualset3
117218	2	403706	13	NULL	NULL	0	NULL	QoL	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference in QoL was found between patients with PPMS and those with secondary progressive MS. The Italian FAMS questionnaire is a valid measure to assess the QoL concerns of patients with MS. FAMS is also easy to administer and is well accepted by patients .
	manualset3
117219	3	403706	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference in QoL was found between patients with PPMS and those with secondary progressive MS. The Italian FAMS questionnaire is a valid measure to assess the QoL concerns of patients with MS. FAMS is also easy to administer and is well accepted by patients .
	manualset3
117220	4	403706	13	NULL	NULL	0	NULL	PPMS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference in QoL was found between patients with PPMS and those with secondary progressive MS. The Italian FAMS questionnaire is a valid measure to assess the QoL concerns of patients with MS. FAMS is also easy to administer and is well accepted by patients .
	manualset3
117221	5	403706	13	NULL	NULL	0	NULL	secondary progressive MS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference in QoL was found between patients with PPMS and those with secondary progressive MS. The Italian FAMS questionnaire is a valid measure to assess the QoL concerns of patients with MS. FAMS is also easy to administer and is well accepted by patients .
	manualset3
117222	6	403706	13	NULL	NULL	0	NULL	Italian FAMS questionnaire 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference in QoL was found between patients with PPMS and those with secondary progressive MS. The Italian FAMS questionnaire is a valid measure to assess the QoL concerns of patients with MS. FAMS is also easy to administer and is well accepted by patients .
	manualset3
117223	7	403706	13	NULL	NULL	0	NULL	measure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference in QoL was found between patients with PPMS and those with secondary progressive MS. The Italian FAMS questionnaire is a valid measure to assess the QoL concerns of patients with MS. FAMS is also easy to administer and is well accepted by patients .
	manualset3
117224	8	403706	13	NULL	NULL	0	NULL	QoL 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference in QoL was found between patients with PPMS and those with secondary progressive MS. The Italian FAMS questionnaire is a valid measure to assess the QoL concerns of patients with MS. FAMS is also easy to administer and is well accepted by patients .
	manualset3
117225	9	403706	13	NULL	NULL	0	NULL	concerns 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference in QoL was found between patients with PPMS and those with secondary progressive MS. The Italian FAMS questionnaire is a valid measure to assess the QoL concerns of patients with MS. FAMS is also easy to administer and is well accepted by patients .
	manualset3
117226	10	403706	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference in QoL was found between patients with PPMS and those with secondary progressive MS. The Italian FAMS questionnaire is a valid measure to assess the QoL concerns of patients with MS. FAMS is also easy to administer and is well accepted by patients .
	manualset3
117227	11	403706	13	NULL	NULL	0	NULL	MS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference in QoL was found between patients with PPMS and those with secondary progressive MS. The Italian FAMS questionnaire is a valid measure to assess the QoL concerns of patients with MS. FAMS is also easy to administer and is well accepted by patients .
	manualset3
117228	12	403706	13	NULL	NULL	0	NULL	FAMS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference in QoL was found between patients with PPMS and those with secondary progressive MS. The Italian FAMS questionnaire is a valid measure to assess the QoL concerns of patients with MS. FAMS is also easy to administer and is well accepted by patients .
	manualset3
117229	13	403706	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference in QoL was found between patients with PPMS and those with secondary progressive MS. The Italian FAMS questionnaire is a valid measure to assess the QoL concerns of patients with MS. FAMS is also easy to administer and is well accepted by patients .
	manualset3
117238	1	403707	13	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference in outcome was found between these two methods as judged by the return or not of the patient within one month and his statement that he did or did not get better .
	manualset3
117239	2	403707	13	NULL	NULL	0	NULL	outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference in outcome was found between these two methods as judged by the return or not of the patient within one month and his statement that he did or did not get better .
	manualset3
117241	3	403707	13	NULL	NULL	0	NULL	two methods	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference in outcome was found between these two methods as judged by the return or not of the patient within one month and his statement that he did or did not get better .
	manualset3
117243	4	403707	13	NULL	NULL	0	NULL	return 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference in outcome was found between these two methods as judged by the return or not of the patient within one month and his statement that he did or did not get better .
	manualset3
117244	5	403707	13	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference in outcome was found between these two methods as judged by the return or not of the patient within one month and his statement that he did or did not get better .
	manualset3
117245	6	403707	13	NULL	NULL	0	NULL	one month 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference in outcome was found between these two methods as judged by the return or not of the patient within one month and his statement that he did or did not get better .
	manualset3
117246	7	403707	13	NULL	NULL	0	NULL	statement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference in outcome was found between these two methods as judged by the return or not of the patient within one month and his statement that he did or did not get better .
	manualset3
117247	1	403708	13	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference was evident in the maximum magnitude of inhibition between the extension and flexion conditions .
	manualset3
117248	2	403708	13	NULL	NULL	0	NULL	magnitude	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference was evident in the maximum magnitude of inhibition between the extension and flexion conditions .
	manualset3
117249	3	403708	13	NULL	NULL	0	NULL	inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference was evident in the maximum magnitude of inhibition between the extension and flexion conditions .
	manualset3
117250	4	403708	13	NULL	NULL	0	NULL	extension conditions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference was evident in the maximum magnitude of inhibition between the extension and flexion conditions .
	manualset3
117251	5	403708	13	NULL	NULL	0	NULL	flexion conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No difference was evident in the maximum magnitude of inhibition between the extension and flexion conditions .
	manualset3
117252	1	403709	13	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	No differences were found in fetal biometric measurements recorded at 20 , 24 , 28 , 32 and 36 weeks gestation between fetuses of women who were supplemented with calcium and those who were not .
	manualset3
117253	2	403709	13	NULL	NULL	0	NULL	fetal biometric measurements	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No differences were found in fetal biometric measurements recorded at 20 , 24 , 28 , 32 and 36 weeks gestation between fetuses of women who were supplemented with calcium and those who were not .
	manualset3
117254	3	403709	13	NULL	NULL	0	NULL	20 weeks gestation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No differences were found in fetal biometric measurements recorded at 20 , 24 , 28 , 32 and 36 weeks gestation between fetuses of women who were supplemented with calcium and those who were not .
	manualset3
117255	4	403709	13	NULL	NULL	0	NULL	24 weeks gestation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No differences were found in fetal biometric measurements recorded at 20 , 24 , 28 , 32 and 36 weeks gestation between fetuses of women who were supplemented with calcium and those who were not .
	manualset3
117256	5	403709	13	NULL	NULL	0	NULL	28 weeks gestation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No differences were found in fetal biometric measurements recorded at 20 , 24 , 28 , 32 and 36 weeks gestation between fetuses of women who were supplemented with calcium and those who were not .
	manualset3
117257	6	403709	13	NULL	NULL	0	NULL	32 weeks gestation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No differences were found in fetal biometric measurements recorded at 20 , 24 , 28 , 32 and 36 weeks gestation between fetuses of women who were supplemented with calcium and those who were not .
	manualset3
117258	7	403709	13	NULL	NULL	0	NULL	36 weeks gestation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No differences were found in fetal biometric measurements recorded at 20 , 24 , 28 , 32 and 36 weeks gestation between fetuses of women who were supplemented with calcium and those who were not .
	manualset3
117259	8	403709	13	NULL	NULL	0	NULL	fetuses of women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No differences were found in fetal biometric measurements recorded at 20 , 24 , 28 , 32 and 36 weeks gestation between fetuses of women who were supplemented with calcium and those who were not .
	manualset3
117260	9	403709	13	NULL	NULL	0	NULL	calcium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	No differences were found in fetal biometric measurements recorded at 20 , 24 , 28 , 32 and 36 weeks gestation between fetuses of women who were supplemented with calcium and those who were not .
	manualset3
117261	1	403710	13	NULL	NULL	0	NULL	effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No effects on lymphocytic subpopulations , mixed lymphocyte reaction , the phagocytosis of leucocytes or the production of immunoglobulins were observed .
	manualset3
117262	2	403710	13	NULL	NULL	0	NULL	lymphocytic subpopulations	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	No effects on lymphocytic subpopulations , mixed lymphocyte reaction , the phagocytosis of leucocytes or the production of immunoglobulins were observed .
	manualset3
117263	3	403710	13	NULL	NULL	0	NULL	mixed lymphocyte reaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	No effects on lymphocytic subpopulations , mixed lymphocyte reaction , the phagocytosis of leucocytes or the production of immunoglobulins were observed .
	manualset3
117264	4	403710	13	NULL	NULL	0	NULL	phagocytosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	No effects on lymphocytic subpopulations , mixed lymphocyte reaction , the phagocytosis of leucocytes or the production of immunoglobulins were observed .
	manualset3
117265	5	403710	13	NULL	NULL	0	NULL	leucocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	No effects on lymphocytic subpopulations , mixed lymphocyte reaction , the phagocytosis of leucocytes or the production of immunoglobulins were observed .
	manualset3
117266	6	403710	13	NULL	NULL	0	NULL	production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	No effects on lymphocytic subpopulations , mixed lymphocyte reaction , the phagocytosis of leucocytes or the production of immunoglobulins were observed .
	manualset3
117267	7	403710	13	NULL	NULL	0	NULL	immunoglobulins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No effects on lymphocytic subpopulations , mixed lymphocyte reaction , the phagocytosis of leucocytes or the production of immunoglobulins were observed .
	manualset3
117268	1	403711	13	NULL	NULL	0	NULL	effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No effects were obtained in uptake of glutamate and activity of GAD in the optic tectum .
	manualset3
117269	2	403711	13	NULL	NULL	NULL	NULL	uptake	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	No effects were obtained in uptake of glutamate and activity of GAD in the optic tectum .
	manualset3
117270	3	403711	13	NULL	NULL	0	NULL	glutamate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	No effects were obtained in uptake of glutamate and activity of GAD in the optic tectum .
	manualset3
117271	4	403711	13	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	No effects were obtained in uptake of glutamate and activity of GAD in the optic tectum .
	manualset3
117272	5	403711	13	NULL	NULL	0	NULL	GAD	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	No effects were obtained in uptake of glutamate and activity of GAD in the optic tectum .
	manualset3
117273	6	403711	13	NULL	NULL	0	NULL	optic tectum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	No effects were obtained in uptake of glutamate and activity of GAD in the optic tectum .
	manualset3
117274	1	403712	13	NULL	NULL	0	NULL	evidence 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	No evidence of renal parenchymal pathologies implicated in the etiology of systemic hypertension was observed , therefore , these animals would seem to be suitable models for human essential hypertension .
	manualset3
117275	2	403712	13	NULL	NULL	0	NULL	renal parenchymal pathologies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No evidence of renal parenchymal pathologies implicated in the etiology of systemic hypertension was observed , therefore , these animals would seem to be suitable models for human essential hypertension .
	manualset3
117276	3	403712	13	NULL	NULL	0	NULL	etiology 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No evidence of renal parenchymal pathologies implicated in the etiology of systemic hypertension was observed , therefore , these animals would seem to be suitable models for human essential hypertension .
	manualset3
117277	4	403712	13	NULL	NULL	0	NULL	systemic hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No evidence of renal parenchymal pathologies implicated in the etiology of systemic hypertension was observed , therefore , these animals would seem to be suitable models for human essential hypertension .
	manualset3
117278	5	403712	13	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	No evidence of renal parenchymal pathologies implicated in the etiology of systemic hypertension was observed , therefore , these animals would seem to be suitable models for human essential hypertension .
	manualset3
117279	6	403712	13	NULL	NULL	0	NULL	models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	No evidence of renal parenchymal pathologies implicated in the etiology of systemic hypertension was observed , therefore , these animals would seem to be suitable models for human essential hypertension .
	manualset3
117280	7	403712	13	NULL	NULL	0	NULL	human essential hypertension 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No evidence of renal parenchymal pathologies implicated in the etiology of systemic hypertension was observed , therefore , these animals would seem to be suitable models for human essential hypertension .
	manualset3
117281	1	403713	13	NULL	NULL	0	NULL	appreciation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A comprehensive appreciation of mechanisms regulating epithelial maintenance and repair in pulmonary airways is fundamental to our understanding of tissue remodeling and dysfunction in chronic lung disease .
	manualset3
117282	2	403713	13	NULL	NULL	0	NULL	mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A comprehensive appreciation of mechanisms regulating epithelial maintenance and repair in pulmonary airways is fundamental to our understanding of tissue remodeling and dysfunction in chronic lung disease .
	manualset3
117283	3	403713	13	NULL	NULL	0	NULL	epithelial maintenance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A comprehensive appreciation of mechanisms regulating epithelial maintenance and repair in pulmonary airways is fundamental to our understanding of tissue remodeling and dysfunction in chronic lung disease .
	manualset3
117284	4	403713	13	NULL	NULL	0	NULL	repair	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A comprehensive appreciation of mechanisms regulating epithelial maintenance and repair in pulmonary airways is fundamental to our understanding of tissue remodeling and dysfunction in chronic lung disease .
	manualset3
117285	5	403713	13	NULL	NULL	0	NULL	pulmonary airways	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A comprehensive appreciation of mechanisms regulating epithelial maintenance and repair in pulmonary airways is fundamental to our understanding of tissue remodeling and dysfunction in chronic lung disease .
	manualset3
117286	6	403713	13	NULL	NULL	0	NULL	understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A comprehensive appreciation of mechanisms regulating epithelial maintenance and repair in pulmonary airways is fundamental to our understanding of tissue remodeling and dysfunction in chronic lung disease .
	manualset3
117287	7	403713	13	NULL	NULL	NULL	NULL	tissue remodeling 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A comprehensive appreciation of mechanisms regulating epithelial maintenance and repair in pulmonary airways is fundamental to our understanding of tissue remodeling and dysfunction in chronic lung disease .
	manualset3
117288	8	403713	13	NULL	NULL	0	NULL	dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A comprehensive appreciation of mechanisms regulating epithelial maintenance and repair in pulmonary airways is fundamental to our understanding of tissue remodeling and dysfunction in chronic lung disease .
	manualset3
117289	9	403713	13	NULL	NULL	0	NULL	chronic lung disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A comprehensive appreciation of mechanisms regulating epithelial maintenance and repair in pulmonary airways is fundamental to our understanding of tissue remodeling and dysfunction in chronic lung disease .
	manualset3
117290	1	403714	13	NULL	NULL	0	NULL	functional redundancy	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	No functional redundancy between the genes was observed and we demonstrate that NirBD is exclusively required for assimilatory nitrite ( it does not detoxify nitrite ) and SirA exclusively for assimilatory sulfite reduction .
	manualset3
117291	2	403714	13	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No functional redundancy between the genes was observed and we demonstrate that NirBD is exclusively required for assimilatory nitrite ( it does not detoxify nitrite ) and SirA exclusively for assimilatory sulfite reduction .
	manualset3
117292	3	403714	13	NULL	NULL	NULL	NULL	NirBD	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	No functional redundancy between the genes was observed and we demonstrate that NirBD is exclusively required for assimilatory nitrite ( it does not detoxify nitrite ) and SirA exclusively for assimilatory sulfite reduction .
	manualset3
117293	4	403714	13	NULL	NULL	0	NULL	assimilatory nitrite 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	No functional redundancy between the genes was observed and we demonstrate that NirBD is exclusively required for assimilatory nitrite ( it does not detoxify nitrite ) and SirA exclusively for assimilatory sulfite reduction .
	manualset3
117294	5	403714	13	NULL	NULL	0	NULL	nitrite 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	No functional redundancy between the genes was observed and we demonstrate that NirBD is exclusively required for assimilatory nitrite ( it does not detoxify nitrite ) and SirA exclusively for assimilatory sulfite reduction .
	manualset3
117295	6	403714	13	NULL	NULL	0	NULL	SirA 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	No functional redundancy between the genes was observed and we demonstrate that NirBD is exclusively required for assimilatory nitrite ( it does not detoxify nitrite ) and SirA exclusively for assimilatory sulfite reduction .
	manualset3
117296	7	403714	13	NULL	NULL	NULL	NULL	assimilatory sulfite	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	No functional redundancy between the genes was observed and we demonstrate that NirBD is exclusively required for assimilatory nitrite ( it does not detoxify nitrite ) and SirA exclusively for assimilatory sulfite reduction .
	manualset3
117297	8	403714	13	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No functional redundancy between the genes was observed and we demonstrate that NirBD is exclusively required for assimilatory nitrite ( it does not detoxify nitrite ) and SirA exclusively for assimilatory sulfite reduction .
	manualset3
117298	1	403715	13	NULL	NULL	0	NULL	group differences 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No group differences were noted in male/female ratios , site of implantation , implantation numbers and number of fetuses .
	manualset3
117299	2	403715	13	NULL	NULL	NULL	NULL	male/female ratios	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	No group differences were noted in male/female ratios , site of implantation , implantation numbers and number of fetuses .
	manualset3
117300	3	403715	13	NULL	NULL	0	NULL	site of implantation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No group differences were noted in male/female ratios , site of implantation , implantation numbers and number of fetuses .
	manualset3
117301	4	403715	13	NULL	NULL	0	NULL	implantation numbers	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No group differences were noted in male/female ratios , site of implantation , implantation numbers and number of fetuses .
	manualset3
117302	5	403715	13	NULL	NULL	0	NULL	number of fetuses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No group differences were noted in male/female ratios , site of implantation , implantation numbers and number of fetuses .
	manualset3
117303	1	403716	13	NULL	NULL	0	NULL	gum	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	No gum was chewed for controls .
	manualset3
117304	2	403716	13	NULL	NULL	0	NULL	controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No gum was chewed for controls .
	manualset3
117305	1	403717	13	NULL	NULL	0	NULL	increases	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No increases in body weight , food intake , or fat mass were found .
	manualset3
117306	2	403717	13	NULL	NULL	NULL	NULL	body weight	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	No increases in body weight , food intake , or fat mass were found .
	manualset3
117307	3	403717	13	NULL	NULL	0	NULL	food intake	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	No increases in body weight , food intake , or fat mass were found .
	manualset3
117308	4	403717	13	NULL	NULL	0	NULL	fat mass	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No increases in body weight , food intake , or fat mass were found .
	manualset3
117309	1	403718	13	NULL	NULL	0	NULL	infiltration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	No infiltration was detected in transgenic mice after irradiation and reconstitution with bone marrow cells .
	manualset3
117310	2	403718	13	NULL	NULL	0	NULL	transgenic mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	No infiltration was detected in transgenic mice after irradiation and reconstitution with bone marrow cells .
	manualset3
117311	3	403718	13	NULL	NULL	0	NULL	irradiation 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	No infiltration was detected in transgenic mice after irradiation and reconstitution with bone marrow cells .
	manualset3
117312	4	403718	13	NULL	NULL	0	NULL	reconstitution	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	No infiltration was detected in transgenic mice after irradiation and reconstitution with bone marrow cells .
	manualset3
117313	5	403718	13	NULL	NULL	0	NULL	bone marrow cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	No infiltration was detected in transgenic mice after irradiation and reconstitution with bone marrow cells .
	manualset3
117314	1	403719	13	NULL	NULL	0	NULL	inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No inhibition was found with optimal concentrations of the ionophore or with TPA present during the preincubation .
	manualset3
117315	2	403719	13	NULL	NULL	0	NULL	optimal concentrations 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No inhibition was found with optimal concentrations of the ionophore or with TPA present during the preincubation .
	manualset3
117316	3	403719	13	NULL	NULL	0	NULL	ionophore	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	No inhibition was found with optimal concentrations of the ionophore or with TPA present during the preincubation .
	manualset3
117317	4	403719	13	NULL	NULL	0	NULL	TPA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	No inhibition was found with optimal concentrations of the ionophore or with TPA present during the preincubation .
	manualset3
117318	5	403719	13	NULL	NULL	0	NULL	preincubation	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	No inhibition was found with optimal concentrations of the ionophore or with TPA present during the preincubation .
	manualset3
117319	1	403720	13	NULL	NULL	0	NULL	interference 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No interference was encountered with isoflurane , desflurane , and sevoflurane when the CAM was set to the `` G '' mode , although extremely high ( nonclinical ) concentrations of halothane and methoxyflurane yielded a weakly positive bar response .
	manualset3
117320	2	403720	13	NULL	NULL	0	NULL	isoflurane	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	No interference was encountered with isoflurane , desflurane , and sevoflurane when the CAM was set to the `` G '' mode , although extremely high ( nonclinical ) concentrations of halothane and methoxyflurane yielded a weakly positive bar response .
	manualset3
117321	3	403720	13	NULL	NULL	0	NULL	desflurane	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	No interference was encountered with isoflurane , desflurane , and sevoflurane when the CAM was set to the `` G '' mode , although extremely high ( nonclinical ) concentrations of halothane and methoxyflurane yielded a weakly positive bar response .
	manualset3
117322	4	403720	13	NULL	NULL	0	NULL	sevoflurane	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	No interference was encountered with isoflurane , desflurane , and sevoflurane when the CAM was set to the `` G '' mode , although extremely high ( nonclinical ) concentrations of halothane and methoxyflurane yielded a weakly positive bar response .
	manualset3
117323	5	403720	13	NULL	NULL	NULL	NULL	CAM	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	No interference was encountered with isoflurane , desflurane , and sevoflurane when the CAM was set to the `` G '' mode , although extremely high ( nonclinical ) concentrations of halothane and methoxyflurane yielded a weakly positive bar response .
	manualset3
117324	6	403720	13	NULL	NULL	0	NULL	`` G '' mode	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No interference was encountered with isoflurane , desflurane , and sevoflurane when the CAM was set to the `` G '' mode , although extremely high ( nonclinical ) concentrations of halothane and methoxyflurane yielded a weakly positive bar response .
	manualset3
117325	7	403720	13	NULL	NULL	0	NULL	concentrations 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No interference was encountered with isoflurane , desflurane , and sevoflurane when the CAM was set to the `` G '' mode , although extremely high ( nonclinical ) concentrations of halothane and methoxyflurane yielded a weakly positive bar response .
	manualset3
117326	8	403720	13	NULL	NULL	0	NULL	halothane	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	No interference was encountered with isoflurane , desflurane , and sevoflurane when the CAM was set to the `` G '' mode , although extremely high ( nonclinical ) concentrations of halothane and methoxyflurane yielded a weakly positive bar response .
	manualset3
117327	9	403720	13	NULL	NULL	0	NULL	methoxyflurane	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	No interference was encountered with isoflurane , desflurane , and sevoflurane when the CAM was set to the `` G '' mode , although extremely high ( nonclinical ) concentrations of halothane and methoxyflurane yielded a weakly positive bar response .
	manualset3
117328	10	403720	13	NULL	NULL	0	NULL	bar response	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No interference was encountered with isoflurane , desflurane , and sevoflurane when the CAM was set to the `` G '' mode , although extremely high ( nonclinical ) concentrations of halothane and methoxyflurane yielded a weakly positive bar response .
	manualset3
117329	1	403721	13	NULL	NULL	0	NULL	miRNA screen	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A comprehensive miRNA screen showed the differential regulation of a number of cellular miRNAs during HCMV latency in CD34 ( + ) progenitor cells .
	manualset3
117330	2	403721	13	NULL	NULL	0	NULL	regulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A comprehensive miRNA screen showed the differential regulation of a number of cellular miRNAs during HCMV latency in CD34 ( + ) progenitor cells .
	manualset3
117331	3	403721	13	NULL	NULL	0	NULL	number	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A comprehensive miRNA screen showed the differential regulation of a number of cellular miRNAs during HCMV latency in CD34 ( + ) progenitor cells .
	manualset3
117332	4	403721	13	NULL	NULL	0	NULL	cellular miRNAs 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A comprehensive miRNA screen showed the differential regulation of a number of cellular miRNAs during HCMV latency in CD34 ( + ) progenitor cells .
	manualset3
117333	5	403721	13	NULL	NULL	0	NULL	HCMV latency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A comprehensive miRNA screen showed the differential regulation of a number of cellular miRNAs during HCMV latency in CD34 ( + ) progenitor cells .
	manualset3
117334	6	403721	13	NULL	NULL	0	NULL	CD34 ( + ) progenitor cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A comprehensive miRNA screen showed the differential regulation of a number of cellular miRNAs during HCMV latency in CD34 ( + ) progenitor cells .
	manualset3
117335	1	403722	13	NULL	NULL	0	NULL	40 contacts 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No new diseased were found among the 40 contacts to whom chemoprophylaxis was applied .
	manualset3
117336	2	403722	13	NULL	NULL	0	NULL	chemoprophylaxis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	No new diseased were found among the 40 contacts to whom chemoprophylaxis was applied .
	manualset3
117337	1	403723	13	NULL	NULL	0	NULL	technique of thoracotomy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	No one technique of thoracotomy has been shown to reduce the incidence of chronic postthoracotomy pain .
	manualset3
117338	2	403723	13	NULL	NULL	0	NULL	incidence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No one technique of thoracotomy has been shown to reduce the incidence of chronic postthoracotomy pain .
	manualset3
117339	3	403723	13	NULL	NULL	0	NULL	chronic postthoracotomy pain 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No one technique of thoracotomy has been shown to reduce the incidence of chronic postthoracotomy pain .
	manualset3
117340	1	403724	13	NULL	NULL	0	NULL	transposition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No other local transposition would have achieved this goal , due to the lack of volume and mobility .
	manualset3
117341	2	403724	13	NULL	NULL	0	NULL	goal 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No other local transposition would have achieved this goal , due to the lack of volume and mobility .
	manualset3
117342	3	403724	13	NULL	NULL	0	NULL	lack of volume	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No other local transposition would have achieved this goal , due to the lack of volume and mobility .
	manualset3
117343	4	403724	13	NULL	NULL	0	NULL	mobility	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No other local transposition would have achieved this goal , due to the lack of volume and mobility .
	manualset3
117344	1	403725	13	NULL	NULL	0	NULL	treatment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	No other treatment was associated with IgG .
	manualset3
117345	2	403725	13	NULL	NULL	0	NULL	IgG	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No other treatment was associated with IgG .
	manualset3
117346	1	403726	13	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	No patient experienced gastric perforation or bleeding during CHT .
	manualset3
117347	2	403726	13	NULL	NULL	0	NULL	gastric perforation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No patient experienced gastric perforation or bleeding during CHT .
	manualset3
117348	3	403726	13	NULL	NULL	0	NULL	bleeding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No patient experienced gastric perforation or bleeding during CHT .
	manualset3
117349	4	403726	13	NULL	NULL	0	NULL	CHT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	No patient experienced gastric perforation or bleeding during CHT .
	manualset3
117350	1	403727	13	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A comprehensive review of the medical literature was conducted and original research articles pertaining to RLS were evaluated .
	manualset3
117351	2	403727	13	NULL	NULL	0	NULL	medical literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A comprehensive review of the medical literature was conducted and original research articles pertaining to RLS were evaluated .
	manualset3
117352	3	403727	13	NULL	NULL	0	NULL	original research articles	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A comprehensive review of the medical literature was conducted and original research articles pertaining to RLS were evaluated .
	manualset3
117353	4	403727	13	NULL	NULL	0	NULL	RLS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A comprehensive review of the medical literature was conducted and original research articles pertaining to RLS were evaluated .
	manualset3
117354	1	403728	13	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	No patient recovered to normal electrophysiology in the severe group .
	manualset3
117355	2	403728	13	NULL	NULL	0	NULL	normal electrophysiology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No patient recovered to normal electrophysiology in the severe group .
	manualset3
117356	3	403728	13	NULL	NULL	0	NULL	severe group 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No patient recovered to normal electrophysiology in the severe group .
	manualset3
117357	1	403729	13	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	No patient who underwent transplantation for CC had histologic evidence of cirrhosis on last evaluable biopsy , compared with 2 % of patients who underwent transplantation for AC and 16 % of patients who underwent transplantation for HCV ( Chi-squared = 13.053 , P = .0015 ) .
	manualset3
117358	2	403729	13	NULL	NULL	0	NULL	transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	No patient who underwent transplantation for CC had histologic evidence of cirrhosis on last evaluable biopsy , compared with 2 % of patients who underwent transplantation for AC and 16 % of patients who underwent transplantation for HCV ( Chi-squared = 13.053 , P = .0015 ) .
	manualset3
117359	3	403729	13	NULL	NULL	0	NULL	CC	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No patient who underwent transplantation for CC had histologic evidence of cirrhosis on last evaluable biopsy , compared with 2 % of patients who underwent transplantation for AC and 16 % of patients who underwent transplantation for HCV ( Chi-squared = 13.053 , P = .0015 ) .
	manualset3
117360	4	403729	13	NULL	NULL	0	NULL	histologic evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No patient who underwent transplantation for CC had histologic evidence of cirrhosis on last evaluable biopsy , compared with 2 % of patients who underwent transplantation for AC and 16 % of patients who underwent transplantation for HCV ( Chi-squared = 13.053 , P = .0015 ) .
	manualset3
117361	5	403729	13	NULL	NULL	0	NULL	cirrhosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No patient who underwent transplantation for CC had histologic evidence of cirrhosis on last evaluable biopsy , compared with 2 % of patients who underwent transplantation for AC and 16 % of patients who underwent transplantation for HCV ( Chi-squared = 13.053 , P = .0015 ) .
	manualset3
117362	6	403729	13	NULL	NULL	0	NULL	evaluable biopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	No patient who underwent transplantation for CC had histologic evidence of cirrhosis on last evaluable biopsy , compared with 2 % of patients who underwent transplantation for AC and 16 % of patients who underwent transplantation for HCV ( Chi-squared = 13.053 , P = .0015 ) .
	manualset3
117363	7	403729	13	NULL	NULL	0	NULL	2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No patient who underwent transplantation for CC had histologic evidence of cirrhosis on last evaluable biopsy , compared with 2 % of patients who underwent transplantation for AC and 16 % of patients who underwent transplantation for HCV ( Chi-squared = 13.053 , P = .0015 ) .
	manualset3
117364	8	403729	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No patient who underwent transplantation for CC had histologic evidence of cirrhosis on last evaluable biopsy , compared with 2 % of patients who underwent transplantation for AC and 16 % of patients who underwent transplantation for HCV ( Chi-squared = 13.053 , P = .0015 ) .
	manualset3
117365	9	403729	13	NULL	NULL	0	NULL	transplantation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	No patient who underwent transplantation for CC had histologic evidence of cirrhosis on last evaluable biopsy , compared with 2 % of patients who underwent transplantation for AC and 16 % of patients who underwent transplantation for HCV ( Chi-squared = 13.053 , P = .0015 ) .
	manualset3
117366	10	403729	13	NULL	NULL	0	NULL	AC	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No patient who underwent transplantation for CC had histologic evidence of cirrhosis on last evaluable biopsy , compared with 2 % of patients who underwent transplantation for AC and 16 % of patients who underwent transplantation for HCV ( Chi-squared = 13.053 , P = .0015 ) .
	manualset3
117367	11	403729	13	NULL	NULL	0	NULL	16 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No patient who underwent transplantation for CC had histologic evidence of cirrhosis on last evaluable biopsy , compared with 2 % of patients who underwent transplantation for AC and 16 % of patients who underwent transplantation for HCV ( Chi-squared = 13.053 , P = .0015 ) .
	manualset3
117368	12	403729	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No patient who underwent transplantation for CC had histologic evidence of cirrhosis on last evaluable biopsy , compared with 2 % of patients who underwent transplantation for AC and 16 % of patients who underwent transplantation for HCV ( Chi-squared = 13.053 , P = .0015 ) .
	manualset3
117369	13	403729	13	NULL	NULL	0	NULL	transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	No patient who underwent transplantation for CC had histologic evidence of cirrhosis on last evaluable biopsy , compared with 2 % of patients who underwent transplantation for AC and 16 % of patients who underwent transplantation for HCV ( Chi-squared = 13.053 , P = .0015 ) .
	manualset3
117370	14	403729	13	NULL	NULL	0	NULL	HCV	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No patient who underwent transplantation for CC had histologic evidence of cirrhosis on last evaluable biopsy , compared with 2 % of patients who underwent transplantation for AC and 16 % of patients who underwent transplantation for HCV ( Chi-squared = 13.053 , P = .0015 ) .
	manualset3
117371	15	403729	13	NULL	NULL	0	NULL	Chi-squared = 13.053 , P = .0015 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No patient who underwent transplantation for CC had histologic evidence of cirrhosis on last evaluable biopsy , compared with 2 % of patients who underwent transplantation for AC and 16 % of patients who underwent transplantation for HCV ( Chi-squared = 13.053 , P = .0015 ) .
	manualset3
117372	1	403730	13	NULL	NULL	0	NULL	preferential effect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No preferential effect was shown for either the high carbohydrate or high protein diet choice .
	manualset3
117373	2	403730	13	NULL	NULL	NULL	NULL	high carbohydrate diet 	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	No preferential effect was shown for either the high carbohydrate or high protein diet choice .
	manualset3
117374	3	403730	13	NULL	NULL	0	NULL	high protein diet 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	No preferential effect was shown for either the high carbohydrate or high protein diet choice .
	manualset3
117375	4	403730	13	NULL	NULL	0	NULL	choice	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	No preferential effect was shown for either the high carbohydrate or high protein diet choice .
	manualset3
117376	1	403731	13	NULL	NULL	0	NULL	changes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No pronounced changes in the blood concentrations of cholesterol , phospholipids or fatty acid esters were observed .
	manualset3
117377	2	403731	13	NULL	NULL	0	NULL	blood concentrations of cholesterol 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No pronounced changes in the blood concentrations of cholesterol , phospholipids or fatty acid esters were observed .
	manualset3
117378	3	403731	13	NULL	NULL	NULL	NULL	blood concentrations of phospholipids	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	No pronounced changes in the blood concentrations of cholesterol , phospholipids or fatty acid esters were observed .
	manualset3
117379	4	403731	13	NULL	NULL	0	NULL	blood concentrations of fatty acid esters	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No pronounced changes in the blood concentrations of cholesterol , phospholipids or fatty acid esters were observed .
	manualset3
117380	1	403732	13	NULL	NULL	0	NULL	Biological properties 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Biological properties of the dermopathic bovine herpes ( Allerton-mammillitis ) virus ) .
	manualset3
117381	2	403732	13	NULL	NULL	0	NULL	dermopathic bovine herpes ( Allerton-mammillitis ) virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Biological properties of the dermopathic bovine herpes ( Allerton-mammillitis ) virus ) .
	manualset3
117382	1	403733	13	NULL	NULL	0	NULL	reaction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No reaction to the highest dose of UVA used for phototesting occurred in 16 % of cases ; the dose of 8-MOP was significantly associated with non-response .
	manualset3
117383	2	403733	13	NULL	NULL	0	NULL	highest dose of UVA 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	No reaction to the highest dose of UVA used for phototesting occurred in 16 % of cases ; the dose of 8-MOP was significantly associated with non-response .
	manualset3
117384	3	403733	13	NULL	NULL	0	NULL	16 % of cases 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No reaction to the highest dose of UVA used for phototesting occurred in 16 % of cases ; the dose of 8-MOP was significantly associated with non-response .
	manualset3
117385	4	403733	13	NULL	NULL	0	NULL	dose of 8-MOP	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	No reaction to the highest dose of UVA used for phototesting occurred in 16 % of cases ; the dose of 8-MOP was significantly associated with non-response .
	manualset3
117386	1	403734	13	NULL	NULL	0	NULL	reactivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No reactivity was observed with TR from bacteria , yeast or rat and only a slight reaction was obtained with TR from horse .
	manualset3
117387	2	403734	13	NULL	NULL	0	NULL	TR 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	No reactivity was observed with TR from bacteria , yeast or rat and only a slight reaction was obtained with TR from horse .
	manualset3
117388	3	403734	13	NULL	NULL	0	NULL	bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	No reactivity was observed with TR from bacteria , yeast or rat and only a slight reaction was obtained with TR from horse .
	manualset3
117389	4	403734	13	NULL	NULL	0	NULL	yeast	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	No reactivity was observed with TR from bacteria , yeast or rat and only a slight reaction was obtained with TR from horse .
	manualset3
117390	5	403734	13	NULL	NULL	0	NULL	rat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	No reactivity was observed with TR from bacteria , yeast or rat and only a slight reaction was obtained with TR from horse .
	manualset3
117391	6	403734	13	NULL	NULL	0	NULL	reaction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No reactivity was observed with TR from bacteria , yeast or rat and only a slight reaction was obtained with TR from horse .
	manualset3
117392	7	403734	13	NULL	NULL	0	NULL	TR 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	No reactivity was observed with TR from bacteria , yeast or rat and only a slight reaction was obtained with TR from horse .
	manualset3
117393	8	403734	13	NULL	NULL	0	NULL	horse	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	No reactivity was observed with TR from bacteria , yeast or rat and only a slight reaction was obtained with TR from horse .
	manualset3
117394	1	403735	13	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	No relationship is found between nursing wages and a new monopsony measure of mobility , but support for new monopsony is found for women elsewhere in the labor market .
	manualset3
117395	2	403735	13	NULL	NULL	0	NULL	wages	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No relationship is found between nursing wages and a new monopsony measure of mobility , but support for new monopsony is found for women elsewhere in the labor market .
	manualset3
117396	3	403735	13	NULL	NULL	0	NULL	monopsony measure	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No relationship is found between nursing wages and a new monopsony measure of mobility , but support for new monopsony is found for women elsewhere in the labor market .
	manualset3
117397	4	403735	13	NULL	NULL	0	NULL	mobility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No relationship is found between nursing wages and a new monopsony measure of mobility , but support for new monopsony is found for women elsewhere in the labor market .
	manualset3
117398	5	403735	13	NULL	NULL	0	NULL	monopsony	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No relationship is found between nursing wages and a new monopsony measure of mobility , but support for new monopsony is found for women elsewhere in the labor market .
	manualset3
117399	6	403735	13	NULL	NULL	0	NULL	women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No relationship is found between nursing wages and a new monopsony measure of mobility , but support for new monopsony is found for women elsewhere in the labor market .
	manualset3
117400	7	403735	13	NULL	NULL	0	NULL	labor market	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No relationship is found between nursing wages and a new monopsony measure of mobility , but support for new monopsony is found for women elsewhere in the labor market .
	manualset3
117406	1	403736	13	NULL	NULL	0	NULL	sample 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	No sample pre-treatment like extraction , steam distillation , purge and trap etc. ; 2 .
	manualset3
117407	2	403736	13	NULL	NULL	0	NULL	extraction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No sample pre-treatment like extraction , steam distillation , purge and trap etc. ; 2 .
	manualset3
117408	3	403736	13	NULL	NULL	0	NULL	steam distillation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No sample pre-treatment like extraction , steam distillation , purge and trap etc. ; 2 .
	manualset3
117409	4	403736	13	NULL	NULL	0	NULL	purge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No sample pre-treatment like extraction , steam distillation , purge and trap etc. ; 2 .
	manualset3
117410	5	403736	13	NULL	NULL	0	NULL	trap	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No sample pre-treatment like extraction , steam distillation , purge and trap etc. ; 2 .
	manualset3
117411	1	403737	13	NULL	NULL	0	NULL	serious side-effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No serious side-effects were reported and interventions were generally popular ; ITNs were the most popular , followed by residual spraying and then impregnated chaddars .
	manualset3
117412	2	403737	13	NULL	NULL	NULL	NULL	interventions	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	No serious side-effects were reported and interventions were generally popular ; ITNs were the most popular , followed by residual spraying and then impregnated chaddars .
	manualset3
117414	3	403737	13	NULL	NULL	0	NULL	ITNs	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	No serious side-effects were reported and interventions were generally popular ; ITNs were the most popular , followed by residual spraying and then impregnated chaddars .
	manualset3
117415	4	403737	13	NULL	NULL	0	NULL	residual spraying	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No serious side-effects were reported and interventions were generally popular ; ITNs were the most popular , followed by residual spraying and then impregnated chaddars .
	manualset3
117416	5	403737	13	NULL	NULL	0	NULL	chaddars	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	No serious side-effects were reported and interventions were generally popular ; ITNs were the most popular , followed by residual spraying and then impregnated chaddars .
	manualset3
117430	1	403738	13	NULL	NULL	0	NULL	alterations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant alterations in densities of M1 , M2 or total muscarinic binding sites were observed in any brain structure evaluated at either early or late stages of thiamine deficiency .
	manualset3
117431	2	403738	13	NULL	NULL	0	NULL	densities of M1	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant alterations in densities of M1 , M2 or total muscarinic binding sites were observed in any brain structure evaluated at either early or late stages of thiamine deficiency .
	manualset3
117432	3	403738	13	NULL	NULL	0	NULL	densities of M2	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant alterations in densities of M1 , M2 or total muscarinic binding sites were observed in any brain structure evaluated at either early or late stages of thiamine deficiency .
	manualset3
117433	4	403738	13	NULL	NULL	0	NULL	muscarinic binding sites	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant alterations in densities of M1 , M2 or total muscarinic binding sites were observed in any brain structure evaluated at either early or late stages of thiamine deficiency .
	manualset3
117434	5	403738	13	NULL	NULL	0	NULL	brain structure	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant alterations in densities of M1 , M2 or total muscarinic binding sites were observed in any brain structure evaluated at either early or late stages of thiamine deficiency .
	manualset3
117435	6	403738	13	NULL	NULL	0	NULL	early stages	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant alterations in densities of M1 , M2 or total muscarinic binding sites were observed in any brain structure evaluated at either early or late stages of thiamine deficiency .
	manualset3
117436	7	403738	13	NULL	NULL	0	NULL	late stages 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant alterations in densities of M1 , M2 or total muscarinic binding sites were observed in any brain structure evaluated at either early or late stages of thiamine deficiency .
	manualset3
117437	8	403738	13	NULL	NULL	0	NULL	thiamine deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant alterations in densities of M1 , M2 or total muscarinic binding sites were observed in any brain structure evaluated at either early or late stages of thiamine deficiency .
	manualset3
117438	1	403739	13	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant association was found between MMP-9 expression and herniation grade in patients who were 30-60 years or over 60 years of age .
	manualset3
117439	2	403739	13	NULL	NULL	0	NULL	MMP-9	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant association was found between MMP-9 expression and herniation grade in patients who were 30-60 years or over 60 years of age .
	manualset3
117440	3	403739	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant association was found between MMP-9 expression and herniation grade in patients who were 30-60 years or over 60 years of age .
	manualset3
117441	4	403739	13	NULL	NULL	0	NULL	herniation grade	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant association was found between MMP-9 expression and herniation grade in patients who were 30-60 years or over 60 years of age .
	manualset3
117442	5	403739	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant association was found between MMP-9 expression and herniation grade in patients who were 30-60 years or over 60 years of age .
	manualset3
117443	6	403739	13	NULL	NULL	0	NULL	30-60 years	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant association was found between MMP-9 expression and herniation grade in patients who were 30-60 years or over 60 years of age .
	manualset3
117444	7	403739	13	NULL	NULL	0	NULL	over 60 years of age	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant association was found between MMP-9 expression and herniation grade in patients who were 30-60 years or over 60 years of age .
	manualset3
117445	1	403740	13	NULL	NULL	0	NULL	blue shift	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant blue shift is observed by replacing PPh3 of 1a with PPh2Me to produce Ir ( ppy ) ( PPh2Me ) 2 ( H ) ( Cl ) ( 1aPPh 2Me ) , which displays emission lambda max at 467 and 494 nm .
	manualset3
117446	2	403740	13	NULL	NULL	NULL	NULL	PPh3	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	No significant blue shift is observed by replacing PPh3 of 1a with PPh2Me to produce Ir ( ppy ) ( PPh2Me ) 2 ( H ) ( Cl ) ( 1aPPh 2Me ) , which displays emission lambda max at 467 and 494 nm .
	manualset3
117447	3	403740	13	NULL	NULL	0	NULL	1a 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant blue shift is observed by replacing PPh3 of 1a with PPh2Me to produce Ir ( ppy ) ( PPh2Me ) 2 ( H ) ( Cl ) ( 1aPPh 2Me ) , which displays emission lambda max at 467 and 494 nm .
	manualset3
117448	4	403740	13	NULL	NULL	0	NULL	PPh2Me 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant blue shift is observed by replacing PPh3 of 1a with PPh2Me to produce Ir ( ppy ) ( PPh2Me ) 2 ( H ) ( Cl ) ( 1aPPh 2Me ) , which displays emission lambda max at 467 and 494 nm .
	manualset3
117449	5	403740	13	NULL	NULL	0	NULL	Ir ( ppy ) ( PPh2Me ) 2 ( H ) ( Cl ) ( 1aPPh 2Me )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant blue shift is observed by replacing PPh3 of 1a with PPh2Me to produce Ir ( ppy ) ( PPh2Me ) 2 ( H ) ( Cl ) ( 1aPPh 2Me ) , which displays emission lambda max at 467 and 494 nm .
	manualset3
117450	6	403740	13	NULL	NULL	0	NULL	emission 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant blue shift is observed by replacing PPh3 of 1a with PPh2Me to produce Ir ( ppy ) ( PPh2Me ) 2 ( H ) ( Cl ) ( 1aPPh 2Me ) , which displays emission lambda max at 467 and 494 nm .
	manualset3
117451	7	403740	13	NULL	NULL	0	NULL	lambda max	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant blue shift is observed by replacing PPh3 of 1a with PPh2Me to produce Ir ( ppy ) ( PPh2Me ) 2 ( H ) ( Cl ) ( 1aPPh 2Me ) , which displays emission lambda max at 467 and 494 nm .
	manualset3
117452	8	403740	13	NULL	NULL	0	NULL	467 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant blue shift is observed by replacing PPh3 of 1a with PPh2Me to produce Ir ( ppy ) ( PPh2Me ) 2 ( H ) ( Cl ) ( 1aPPh 2Me ) , which displays emission lambda max at 467 and 494 nm .
	manualset3
117453	9	403740	13	NULL	NULL	0	NULL	494 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant blue shift is observed by replacing PPh3 of 1a with PPh2Me to produce Ir ( ppy ) ( PPh2Me ) 2 ( H ) ( Cl ) ( 1aPPh 2Me ) , which displays emission lambda max at 467 and 494 nm .
	manualset3
117454	1	403741	13	NULL	NULL	0	NULL	SPECT-CT image	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A computer-generated composite SPECT-CT image confirmed the intravascular localization of the radioisotope , and a subsequent CT-guided transthoracic needle biopsy revealed a poorly differentiated adenocarcinoma .
	manualset3
117455	2	403741	13	NULL	NULL	0	NULL	intravascular localization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A computer-generated composite SPECT-CT image confirmed the intravascular localization of the radioisotope , and a subsequent CT-guided transthoracic needle biopsy revealed a poorly differentiated adenocarcinoma .
	manualset3
117456	3	403741	13	NULL	NULL	0	NULL	radioisotope	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A computer-generated composite SPECT-CT image confirmed the intravascular localization of the radioisotope , and a subsequent CT-guided transthoracic needle biopsy revealed a poorly differentiated adenocarcinoma .
	manualset3
117457	4	403741	13	NULL	NULL	0	NULL	CT-guided transthoracic needle biopsy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A computer-generated composite SPECT-CT image confirmed the intravascular localization of the radioisotope , and a subsequent CT-guided transthoracic needle biopsy revealed a poorly differentiated adenocarcinoma .
	manualset3
117458	5	403741	13	NULL	NULL	0	NULL	adenocarcinoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A computer-generated composite SPECT-CT image confirmed the intravascular localization of the radioisotope , and a subsequent CT-guided transthoracic needle biopsy revealed a poorly differentiated adenocarcinoma .
	manualset3
117459	1	403742	13	NULL	NULL	0	NULL	cleavage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant cleavage of protein kinase C delta ( Pkcd ) in vivo , which is a substrate for caspase 3 , was detected , and intact Pkcd was retained in both cell lines for at least 72 h after irradiation .
	manualset3
117460	2	403742	13	NULL	NULL	0	NULL	protein kinase C delta ( Pkcd ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant cleavage of protein kinase C delta ( Pkcd ) in vivo , which is a substrate for caspase 3 , was detected , and intact Pkcd was retained in both cell lines for at least 72 h after irradiation .
	manualset3
117461	3	403742	13	NULL	NULL	0	NULL	substrate	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant cleavage of protein kinase C delta ( Pkcd ) in vivo , which is a substrate for caspase 3 , was detected , and intact Pkcd was retained in both cell lines for at least 72 h after irradiation .
	manualset3
117462	4	403742	13	NULL	NULL	0	NULL	caspase 3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant cleavage of protein kinase C delta ( Pkcd ) in vivo , which is a substrate for caspase 3 , was detected , and intact Pkcd was retained in both cell lines for at least 72 h after irradiation .
	manualset3
117463	5	403742	13	NULL	NULL	0	NULL	Pkcd	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant cleavage of protein kinase C delta ( Pkcd ) in vivo , which is a substrate for caspase 3 , was detected , and intact Pkcd was retained in both cell lines for at least 72 h after irradiation .
	manualset3
117464	6	403742	13	NULL	NULL	0	NULL	cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant cleavage of protein kinase C delta ( Pkcd ) in vivo , which is a substrate for caspase 3 , was detected , and intact Pkcd was retained in both cell lines for at least 72 h after irradiation .
	manualset3
117465	7	403742	13	NULL	NULL	0	NULL	72 h 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant cleavage of protein kinase C delta ( Pkcd ) in vivo , which is a substrate for caspase 3 , was detected , and intact Pkcd was retained in both cell lines for at least 72 h after irradiation .
	manualset3
117466	8	403742	13	NULL	NULL	0	NULL	irradiation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant cleavage of protein kinase C delta ( Pkcd ) in vivo , which is a substrate for caspase 3 , was detected , and intact Pkcd was retained in both cell lines for at least 72 h after irradiation .
	manualset3
117467	1	403743	13	NULL	NULL	0	NULL	clinical deficit 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant clinical deficit subsequent to dividing the anterior part of the body of the corpus callosum could be demonstrated .
	manualset3
117468	2	403743	13	NULL	NULL	0	NULL	anterior part of the body	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant clinical deficit subsequent to dividing the anterior part of the body of the corpus callosum could be demonstrated .
	manualset3
117469	3	403743	13	NULL	NULL	0	NULL	corpus callosum 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant clinical deficit subsequent to dividing the anterior part of the body of the corpus callosum could be demonstrated .
	manualset3
117470	1	403744	13	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant correlation was found between mean size of anterior fontanelle and head circumference or with gestational age of infant ( P0 .05 ) .
	manualset3
117471	2	403744	13	NULL	NULL	0	NULL	mean size	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant correlation was found between mean size of anterior fontanelle and head circumference or with gestational age of infant ( P0 .05 ) .
	manualset3
117472	3	403744	13	NULL	NULL	0	NULL	anterior fontanelle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant correlation was found between mean size of anterior fontanelle and head circumference or with gestational age of infant ( P0 .05 ) .
	manualset3
117473	4	403744	13	NULL	NULL	NULL	NULL	head circumference	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	No significant correlation was found between mean size of anterior fontanelle and head circumference or with gestational age of infant ( P0 .05 ) .
	manualset3
117474	5	403744	13	NULL	NULL	0	NULL	gestational age	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant correlation was found between mean size of anterior fontanelle and head circumference or with gestational age of infant ( P0 .05 ) .
	manualset3
117475	6	403744	13	NULL	NULL	0	NULL	infant 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant correlation was found between mean size of anterior fontanelle and head circumference or with gestational age of infant ( P0 .05 ) .
	manualset3
117476	7	403744	13	NULL	NULL	0	NULL	P0 .05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant correlation was found between mean size of anterior fontanelle and head circumference or with gestational age of infant ( P0 .05 ) .
	manualset3
117479	1	403745	13	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant difference was observed between RA1 and RA2 .
	manualset3
117480	2	403745	13	NULL	NULL	0	NULL	RA1 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant difference was observed between RA1 and RA2 .
	manualset3
117481	3	403745	13	NULL	NULL	0	NULL	RA2	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant difference was observed between RA1 and RA2 .
	manualset3
117482	1	403746	13	NULL	NULL	0	NULL	difference 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant difference was observed between the pattern of hormone secretion during saline alone and after rosiglitazone , as evaluated by two-way analysis of variance ( ANOVA ) .
	manualset3
117483	2	403746	13	NULL	NULL	0	NULL	pattern of hormone secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant difference was observed between the pattern of hormone secretion during saline alone and after rosiglitazone , as evaluated by two-way analysis of variance ( ANOVA ) .
	manualset3
117484	3	403746	13	NULL	NULL	0	NULL	saline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant difference was observed between the pattern of hormone secretion during saline alone and after rosiglitazone , as evaluated by two-way analysis of variance ( ANOVA ) .
	manualset3
117485	4	403746	13	NULL	NULL	0	NULL	rosiglitazone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant difference was observed between the pattern of hormone secretion during saline alone and after rosiglitazone , as evaluated by two-way analysis of variance ( ANOVA ) .
	manualset3
117486	5	403746	13	NULL	NULL	0	NULL	two-way analysis of variance ( ANOVA ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant difference was observed between the pattern of hormone secretion during saline alone and after rosiglitazone , as evaluated by two-way analysis of variance ( ANOVA ) .
	manualset3
117487	1	403747	13	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant difference was observed in IgG antibody levels to pneumococcal polysaccharides between atopic and non-atopic recruits , whereas seropositivity to T. gondii was found to be less frequent among the atopic recruits ( odds ratio , 0.37 ; 95 % CI , 0.17-0 .81 ; P = 0.01 ) .
	manualset3
117488	2	403747	13	NULL	NULL	0	NULL	IgG antibody levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant difference was observed in IgG antibody levels to pneumococcal polysaccharides between atopic and non-atopic recruits , whereas seropositivity to T. gondii was found to be less frequent among the atopic recruits ( odds ratio , 0.37 ; 95 % CI , 0.17-0 .81 ; P = 0.01 ) .
	manualset3
117489	3	403747	13	NULL	NULL	0	NULL	pneumococcal polysaccharides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant difference was observed in IgG antibody levels to pneumococcal polysaccharides between atopic and non-atopic recruits , whereas seropositivity to T. gondii was found to be less frequent among the atopic recruits ( odds ratio , 0.37 ; 95 % CI , 0.17-0 .81 ; P = 0.01 ) .
	manualset3
117491	4	403747	13	NULL	NULL	0	NULL	atopic recruits	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant difference was observed in IgG antibody levels to pneumococcal polysaccharides between atopic and non-atopic recruits , whereas seropositivity to T. gondii was found to be less frequent among the atopic recruits ( odds ratio , 0.37 ; 95 % CI , 0.17-0 .81 ; P = 0.01 ) .
	manualset3
117492	5	403747	13	NULL	NULL	0	NULL	non-atopic recruits	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant difference was observed in IgG antibody levels to pneumococcal polysaccharides between atopic and non-atopic recruits , whereas seropositivity to T. gondii was found to be less frequent among the atopic recruits ( odds ratio , 0.37 ; 95 % CI , 0.17-0 .81 ; P = 0.01 ) .
	manualset3
117493	6	403747	13	NULL	NULL	0	NULL	seropositivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant difference was observed in IgG antibody levels to pneumococcal polysaccharides between atopic and non-atopic recruits , whereas seropositivity to T. gondii was found to be less frequent among the atopic recruits ( odds ratio , 0.37 ; 95 % CI , 0.17-0 .81 ; P = 0.01 ) .
	manualset3
117502	7	403747	13	NULL	NULL	0	NULL	T. gondii	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant difference was observed in IgG antibody levels to pneumococcal polysaccharides between atopic and non-atopic recruits , whereas seropositivity to T. gondii was found to be less frequent among the atopic recruits ( odds ratio , 0.37 ; 95 % CI , 0.17-0 .81 ; P = 0.01 ) .
	manualset3
117504	8	403747	13	NULL	NULL	0	NULL	atopic recruits 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant difference was observed in IgG antibody levels to pneumococcal polysaccharides between atopic and non-atopic recruits , whereas seropositivity to T. gondii was found to be less frequent among the atopic recruits ( odds ratio , 0.37 ; 95 % CI , 0.17-0 .81 ; P = 0.01 ) .
	manualset3
117505	9	403747	13	NULL	NULL	0	NULL	odds ratio , 0.37 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant difference was observed in IgG antibody levels to pneumococcal polysaccharides between atopic and non-atopic recruits , whereas seropositivity to T. gondii was found to be less frequent among the atopic recruits ( odds ratio , 0.37 ; 95 % CI , 0.17-0 .81 ; P = 0.01 ) .
	manualset3
117506	10	403747	13	NULL	NULL	0	NULL	95 % CI , 0.17-0 .81	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant difference was observed in IgG antibody levels to pneumococcal polysaccharides between atopic and non-atopic recruits , whereas seropositivity to T. gondii was found to be less frequent among the atopic recruits ( odds ratio , 0.37 ; 95 % CI , 0.17-0 .81 ; P = 0.01 ) .
	manualset3
117508	11	403747	13	NULL	NULL	0	NULL	P = 0.01 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant difference was observed in IgG antibody levels to pneumococcal polysaccharides between atopic and non-atopic recruits , whereas seropositivity to T. gondii was found to be less frequent among the atopic recruits ( odds ratio , 0.37 ; 95 % CI , 0.17-0 .81 ; P = 0.01 ) .
	manualset3
117511	1	403748	13	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences between the first and second serves were found in the pre-impact racquet head speed and orientation , which was represented as a unit vector perpendicular to the racquet face .
	manualset3
117512	2	403748	13	NULL	NULL	0	NULL	first serve	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences between the first and second serves were found in the pre-impact racquet head speed and orientation , which was represented as a unit vector perpendicular to the racquet face .
	manualset3
117513	3	403748	13	NULL	NULL	0	NULL	second serve	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences between the first and second serves were found in the pre-impact racquet head speed and orientation , which was represented as a unit vector perpendicular to the racquet face .
	manualset3
117514	4	403748	13	NULL	NULL	0	NULL	racquet head speed	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences between the first and second serves were found in the pre-impact racquet head speed and orientation , which was represented as a unit vector perpendicular to the racquet face .
	manualset3
117515	5	403748	13	NULL	NULL	0	NULL	orientation 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences between the first and second serves were found in the pre-impact racquet head speed and orientation , which was represented as a unit vector perpendicular to the racquet face .
	manualset3
117516	6	403748	13	NULL	NULL	0	NULL	unit vector 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences between the first and second serves were found in the pre-impact racquet head speed and orientation , which was represented as a unit vector perpendicular to the racquet face .
	manualset3
117517	7	403748	13	NULL	NULL	0	NULL	racquet face 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences between the first and second serves were found in the pre-impact racquet head speed and orientation , which was represented as a unit vector perpendicular to the racquet face .
	manualset3
117518	1	403749	13	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences in elemental content of placenta and membrane samples were observed except for Ca .
	manualset3
117519	2	403749	13	NULL	NULL	0	NULL	elemental content	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences in elemental content of placenta and membrane samples were observed except for Ca .
	manualset3
117520	3	403749	13	NULL	NULL	0	NULL	placenta	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences in elemental content of placenta and membrane samples were observed except for Ca .
	manualset3
117521	4	403749	13	NULL	NULL	0	NULL	membrane samples	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences in elemental content of placenta and membrane samples were observed except for Ca .
	manualset3
117522	5	403749	13	NULL	NULL	0	NULL	Ca	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences in elemental content of placenta and membrane samples were observed except for Ca .
	manualset3
117523	1	403750	13	NULL	NULL	NULL	NULL	computer data-processing system 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A computer data-processing system in the chemical pathology laboratories of the Royal Postgraduate Medical School at Hammersmith Hospital was described recently .
	manualset3
117524	2	403750	13	NULL	NULL	0	NULL	 chemical pathology laboratories	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A computer data-processing system in the chemical pathology laboratories of the Royal Postgraduate Medical School at Hammersmith Hospital was described recently .
	manualset3
117525	3	403750	13	NULL	NULL	0	NULL	Royal Postgraduate Medical School 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A computer data-processing system in the chemical pathology laboratories of the Royal Postgraduate Medical School at Hammersmith Hospital was described recently .
	manualset3
117526	4	403750	13	NULL	NULL	0	NULL	Hammersmith Hospital 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A computer data-processing system in the chemical pathology laboratories of the Royal Postgraduate Medical School at Hammersmith Hospital was described recently .
	manualset3
117527	1	403751	13	NULL	NULL	0	NULL	differences 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences in the numbers of CL were found between the groups .
	manualset3
117528	2	403751	13	NULL	NULL	0	NULL	numbers 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences in the numbers of CL were found between the groups .
	manualset3
117529	3	403751	13	NULL	NULL	0	NULL	CL	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences in the numbers of CL were found between the groups .
	manualset3
117530	4	403751	13	NULL	NULL	0	NULL	groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences in the numbers of CL were found between the groups .
	manualset3
117531	1	403752	13	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences were demonstrated between the slopes and intercepts of regression lines for adrenaline , noradrenaline and dopamine within either cohort ( ANCOVA ) .
	manualset3
117532	2	403752	13	NULL	NULL	0	NULL	 slopes regression lines	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences were demonstrated between the slopes and intercepts of regression lines for adrenaline , noradrenaline and dopamine within either cohort ( ANCOVA ) .
	manualset3
117533	3	403752	13	NULL	NULL	0	NULL	intercepts of regression lines	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences were demonstrated between the slopes and intercepts of regression lines for adrenaline , noradrenaline and dopamine within either cohort ( ANCOVA ) .
	manualset3
117534	4	403752	13	NULL	NULL	0	NULL	adrenaline	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences were demonstrated between the slopes and intercepts of regression lines for adrenaline , noradrenaline and dopamine within either cohort ( ANCOVA ) .
	manualset3
117535	5	403752	13	NULL	NULL	0	NULL	noradrenaline	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences were demonstrated between the slopes and intercepts of regression lines for adrenaline , noradrenaline and dopamine within either cohort ( ANCOVA ) .
	manualset3
117536	6	403752	13	NULL	NULL	0	NULL	dopamine 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences were demonstrated between the slopes and intercepts of regression lines for adrenaline , noradrenaline and dopamine within either cohort ( ANCOVA ) .
	manualset3
117537	7	403752	13	NULL	NULL	NULL	NULL	cohort	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	No significant differences were demonstrated between the slopes and intercepts of regression lines for adrenaline , noradrenaline and dopamine within either cohort ( ANCOVA ) .
	manualset3
120446	8	403752	13	NULL	NULL	0	NULL	ANCOVA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences were demonstrated between the slopes and intercepts of regression lines for adrenaline , noradrenaline and dopamine within either cohort ( ANCOVA ) .
	manualset3
117545	1	403753	13	NULL	NULL	0	NULL	differences 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences were found between sites in terms of non-enzymatic defenses ( GSHt and NPT ) .
	manualset3
117549	2	403753	13	NULL	NULL	0	NULL	sites 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences were found between sites in terms of non-enzymatic defenses ( GSHt and NPT ) .
	manualset3
117550	3	403753	13	NULL	NULL	0	NULL	terms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences were found between sites in terms of non-enzymatic defenses ( GSHt and NPT ) .
	manualset3
117551	4	403753	13	NULL	NULL	0	NULL	non-enzymatic defenses 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences were found between sites in terms of non-enzymatic defenses ( GSHt and NPT ) .
	manualset3
117552	5	403753	13	NULL	NULL	0	NULL	GSHt 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences were found between sites in terms of non-enzymatic defenses ( GSHt and NPT ) .
	manualset3
117553	6	403753	13	NULL	NULL	0	NULL	NPT	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences were found between sites in terms of non-enzymatic defenses ( GSHt and NPT ) .
	manualset3
117554	1	403754	13	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences were observed in the Km for hexokinase with 2-DG as the substrate in the glioma and normal brain tissue .
	manualset3
117563	2	403754	13	NULL	NULL	0	NULL	Km	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences were observed in the Km for hexokinase with 2-DG as the substrate in the glioma and normal brain tissue .
	manualset3
117565	3	403754	13	NULL	NULL	0	NULL	hexokinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences were observed in the Km for hexokinase with 2-DG as the substrate in the glioma and normal brain tissue .
	manualset3
117569	4	403754	13	NULL	NULL	0	NULL	2-DG	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences were observed in the Km for hexokinase with 2-DG as the substrate in the glioma and normal brain tissue .
	manualset3
117570	5	403754	13	NULL	NULL	0	NULL	substrate	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences were observed in the Km for hexokinase with 2-DG as the substrate in the glioma and normal brain tissue .
	manualset3
117572	6	403754	13	NULL	NULL	0	NULL	glioma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences were observed in the Km for hexokinase with 2-DG as the substrate in the glioma and normal brain tissue .
	manualset3
117574	7	403754	13	NULL	NULL	0	NULL	normal brain tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences were observed in the Km for hexokinase with 2-DG as the substrate in the glioma and normal brain tissue .
	manualset3
117580	1	403755	13	NULL	NULL	0	NULL	differences 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences were observed in the responses to concanavaline A between stages of the cycle .
	manualset3
117581	2	403755	13	NULL	NULL	0	NULL	responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences were observed in the responses to concanavaline A between stages of the cycle .
	manualset3
117582	3	403755	13	NULL	NULL	0	NULL	concanavaline A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences were observed in the responses to concanavaline A between stages of the cycle .
	manualset3
117583	4	403755	13	NULL	NULL	0	NULL	stages of the cycle	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant differences were observed in the responses to concanavaline A between stages of the cycle .
	manualset3
117591	1	403756	13	NULL	NULL	0	NULL	effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant effect of the XbaI genotype on BMD was found at any site .
	manualset3
117592	2	403756	13	NULL	NULL	0	NULL	XbaI genotype	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant effect of the XbaI genotype on BMD was found at any site .
	manualset3
117594	3	403756	13	NULL	NULL	0	NULL	BMD 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant effect of the XbaI genotype on BMD was found at any site .
	manualset3
117602	4	403756	13	NULL	NULL	0	NULL	site 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant effect of the XbaI genotype on BMD was found at any site .
	manualset3
117606	1	403757	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant increase in cells with chromosomal aberrations , polyploidy , or endoreduplication was observed in the cultures analyzed .
	manualset3
117607	2	403757	13	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant increase in cells with chromosomal aberrations , polyploidy , or endoreduplication was observed in the cultures analyzed .
	manualset3
117609	3	403757	13	NULL	NULL	0	NULL	chromosomal aberrations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant increase in cells with chromosomal aberrations , polyploidy , or endoreduplication was observed in the cultures analyzed .
	manualset3
117610	4	403757	13	NULL	NULL	0	NULL	polyploidy	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant increase in cells with chromosomal aberrations , polyploidy , or endoreduplication was observed in the cultures analyzed .
	manualset3
117611	5	403757	13	NULL	NULL	0	NULL	endoreduplication	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant increase in cells with chromosomal aberrations , polyploidy , or endoreduplication was observed in the cultures analyzed .
	manualset3
117613	6	403757	13	NULL	NULL	0	NULL	cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant increase in cells with chromosomal aberrations , polyploidy , or endoreduplication was observed in the cultures analyzed .
	manualset3
117622	1	403758	13	NULL	NULL	0	NULL	loss 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant loss of middle molecular weight hormones attached to other carrier proteins was observed .
	manualset3
117623	2	403758	13	NULL	NULL	0	NULL	middle molecular weight hormones 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant loss of middle molecular weight hormones attached to other carrier proteins was observed .
	manualset3
117624	3	403758	13	NULL	NULL	0	NULL	carrier proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant loss of middle molecular weight hormones attached to other carrier proteins was observed .
	manualset3
117629	1	403759	13	NULL	NULL	0	NULL	significant sleep change 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant sleep change was observed on the withdrawal night .
	manualset3
117636	2	403759	13	NULL	NULL	0	NULL	withdrawal 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant sleep change was observed on the withdrawal night .
	manualset3
117637	3	403759	13	NULL	NULL	0	NULL	night	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant sleep change was observed on the withdrawal night .
	manualset3
117640	1	403760	13	NULL	NULL	0	NULL	specific autoantibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No specific autoantibodies to human tissue extracts were demonstrable by complement fixation or by the collodion particle technique .
	manualset3
117641	2	403760	13	NULL	NULL	0	NULL	human tissue extracts 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	No specific autoantibodies to human tissue extracts were demonstrable by complement fixation or by the collodion particle technique .
	manualset3
117643	3	403760	13	NULL	NULL	0	NULL	complement fixation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	No specific autoantibodies to human tissue extracts were demonstrable by complement fixation or by the collodion particle technique .
	manualset3
117644	4	403760	13	NULL	NULL	0	NULL	collodion particle technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	No specific autoantibodies to human tissue extracts were demonstrable by complement fixation or by the collodion particle technique .
	manualset3
117645	1	403761	13	NULL	NULL	0	NULL	computer program 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A computer program is described , by which data on reproduction ( data on calving , oestrus and insemination , pregnancy diagnosis ) in dairy herds may be processed .
	manualset3
117647	2	403761	13	NULL	NULL	NULL	NULL	data on reproduction	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A computer program is described , by which data on reproduction ( data on calving , oestrus and insemination , pregnancy diagnosis ) in dairy herds may be processed .
	manualset3
117649	3	403761	13	NULL	NULL	0	NULL	data on calving	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A computer program is described , by which data on reproduction ( data on calving , oestrus and insemination , pregnancy diagnosis ) in dairy herds may be processed .
	manualset3
117652	4	403761	13	NULL	NULL	0	NULL	data on oestrus	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A computer program is described , by which data on reproduction ( data on calving , oestrus and insemination , pregnancy diagnosis ) in dairy herds may be processed .
	manualset3
117654	5	403761	13	NULL	NULL	0	NULL	data on insemination	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A computer program is described , by which data on reproduction ( data on calving , oestrus and insemination , pregnancy diagnosis ) in dairy herds may be processed .
	manualset3
117655	6	403761	13	NULL	NULL	0	NULL	pregnancy diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A computer program is described , by which data on reproduction ( data on calving , oestrus and insemination , pregnancy diagnosis ) in dairy herds may be processed .
	manualset3
117656	7	403761	13	NULL	NULL	0	NULL	dairy herds	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A computer program is described , by which data on reproduction ( data on calving , oestrus and insemination , pregnancy diagnosis ) in dairy herds may be processed .
	manualset3
117657	1	403762	13	NULL	NULL	0	NULL	sperm 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	No sperm was detected in testes or epididymes .
	manualset3
117659	2	403762	13	NULL	NULL	0	NULL	testes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	No sperm was detected in testes or epididymes .
	manualset3
117660	3	403762	13	NULL	NULL	0	NULL	epididymes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	No sperm was detected in testes or epididymes .
	manualset3
117667	1	403763	13	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	No statistically significant differences between the recanalized group after the administration of intracoronary urokinase and the control group were found at each coronary lesion .
	manualset3
117668	2	403763	13	NULL	NULL	0	NULL	recanalized group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No statistically significant differences between the recanalized group after the administration of intracoronary urokinase and the control group were found at each coronary lesion .
	manualset3
117669	3	403763	13	NULL	NULL	0	NULL	administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	No statistically significant differences between the recanalized group after the administration of intracoronary urokinase and the control group were found at each coronary lesion .
	manualset3
117670	4	403763	13	NULL	NULL	0	NULL	 intracoronary urokinase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	No statistically significant differences between the recanalized group after the administration of intracoronary urokinase and the control group were found at each coronary lesion .
	manualset3
117671	5	403763	13	NULL	NULL	0	NULL	control group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No statistically significant differences between the recanalized group after the administration of intracoronary urokinase and the control group were found at each coronary lesion .
	manualset3
117672	6	403763	13	NULL	NULL	0	NULL	coronary lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No statistically significant differences between the recanalized group after the administration of intracoronary urokinase and the control group were found at each coronary lesion .
	manualset3
117674	1	403764	13	NULL	NULL	0	NULL	stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	No stimulation of guanylate cyclase activity by gastrin was detected in the dispersed gastric corporal mucosal cells .
	manualset3
117675	2	403764	13	NULL	NULL	0	NULL	guanylate cyclase activity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	No stimulation of guanylate cyclase activity by gastrin was detected in the dispersed gastric corporal mucosal cells .
	manualset3
117676	3	403764	13	NULL	NULL	0	NULL	gastrin 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	No stimulation of guanylate cyclase activity by gastrin was detected in the dispersed gastric corporal mucosal cells .
	manualset3
117677	4	403764	13	NULL	NULL	0	NULL	gastric corporal mucosal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	No stimulation of guanylate cyclase activity by gastrin was detected in the dispersed gastric corporal mucosal cells .
	manualset3
117678	1	403765	13	NULL	NULL	0	NULL	changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No such significant changes as fibrosis , vacuolation , and atrophy of acinar cells were observed in the submandibular and sublingual glands of the experimental animals .
	manualset3
117679	2	403765	13	NULL	NULL	0	NULL	fibrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No such significant changes as fibrosis , vacuolation , and atrophy of acinar cells were observed in the submandibular and sublingual glands of the experimental animals .
	manualset3
117680	3	403765	13	NULL	NULL	0	NULL	vacuolation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No such significant changes as fibrosis , vacuolation , and atrophy of acinar cells were observed in the submandibular and sublingual glands of the experimental animals .
	manualset3
117681	4	403765	13	NULL	NULL	0	NULL	atrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No such significant changes as fibrosis , vacuolation , and atrophy of acinar cells were observed in the submandibular and sublingual glands of the experimental animals .
	manualset3
117682	5	403765	13	NULL	NULL	0	NULL	acinar cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	No such significant changes as fibrosis , vacuolation , and atrophy of acinar cells were observed in the submandibular and sublingual glands of the experimental animals .
	manualset3
117683	6	403765	13	NULL	NULL	0	NULL	submandibular glands	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	No such significant changes as fibrosis , vacuolation , and atrophy of acinar cells were observed in the submandibular and sublingual glands of the experimental animals .
	manualset3
117684	7	403765	13	NULL	NULL	0	NULL	sublingual glands	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	No such significant changes as fibrosis , vacuolation , and atrophy of acinar cells were observed in the submandibular and sublingual glands of the experimental animals .
	manualset3
117685	8	403765	13	NULL	NULL	0	NULL	experimental animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	No such significant changes as fibrosis , vacuolation , and atrophy of acinar cells were observed in the submandibular and sublingual glands of the experimental animals .
	manualset3
117713	1	403766	13	NULL	NULL	0	NULL	toxicity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No toxicity has been demonstrated in man , although the dose for laxation ( to be distinguished from diarrhoea ) is approximately 90 g/day ( v. sorbitol at 70 g/day ) .
	manualset3
117714	2	403766	13	NULL	NULL	0	NULL	man	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	No toxicity has been demonstrated in man , although the dose for laxation ( to be distinguished from diarrhoea ) is approximately 90 g/day ( v. sorbitol at 70 g/day ) .
	manualset3
117715	3	403766	13	NULL	NULL	0	NULL	dose for laxation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	No toxicity has been demonstrated in man , although the dose for laxation ( to be distinguished from diarrhoea ) is approximately 90 g/day ( v. sorbitol at 70 g/day ) .
	manualset3
117716	4	403766	13	NULL	NULL	0	NULL	diarrhoea	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No toxicity has been demonstrated in man , although the dose for laxation ( to be distinguished from diarrhoea ) is approximately 90 g/day ( v. sorbitol at 70 g/day ) .
	manualset3
117717	5	403766	13	NULL	NULL	0	NULL	90 g/day	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No toxicity has been demonstrated in man , although the dose for laxation ( to be distinguished from diarrhoea ) is approximately 90 g/day ( v. sorbitol at 70 g/day ) .
	manualset3
117718	6	403766	13	NULL	NULL	0	NULL	sorbitol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	No toxicity has been demonstrated in man , although the dose for laxation ( to be distinguished from diarrhoea ) is approximately 90 g/day ( v. sorbitol at 70 g/day ) .
	manualset3
117719	7	403766	13	NULL	NULL	0	NULL	70 g/day 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No toxicity has been demonstrated in man , although the dose for laxation ( to be distinguished from diarrhoea ) is approximately 90 g/day ( v. sorbitol at 70 g/day ) .
	manualset3
117720	1	403767	13	NULL	NULL	0	NULL	toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No toxicity was observed for MWNTs alone .
	manualset3
117721	2	403767	13	NULL	NULL	0	NULL	MWNTs	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	No toxicity was observed for MWNTs alone .
	manualset3
117722	1	403768	13	NULL	NULL	0	NULL	transcript	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	No transcript was detected in the lymphoblastoid cell lines MOLT-4 and BALM-1 .
	manualset3
117723	2	403768	13	NULL	NULL	0	NULL	lymphoblastoid cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	No transcript was detected in the lymphoblastoid cell lines MOLT-4 and BALM-1 .
	manualset3
117724	3	403768	13	NULL	NULL	0	NULL	MOLT-4 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	No transcript was detected in the lymphoblastoid cell lines MOLT-4 and BALM-1 .
	manualset3
117725	4	403768	13	NULL	NULL	0	NULL	BALM-1	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	No transcript was detected in the lymphoblastoid cell lines MOLT-4 and BALM-1 .
	manualset3
117726	1	403769	13	NULL	NULL	0	NULL	translocations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	No translocations involving bcl-2 and the immunoglobulin heavy chain gene were identified ; two cases had translocations involving the bcl-1 and the immunoglobulin heavy chain genes .
	manualset3
117727	2	403769	13	NULL	NULL	0	NULL	bcl-2	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	No translocations involving bcl-2 and the immunoglobulin heavy chain gene were identified ; two cases had translocations involving the bcl-1 and the immunoglobulin heavy chain genes .
	manualset3
117728	3	403769	13	NULL	NULL	0	NULL	immunoglobulin heavy chain gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	No translocations involving bcl-2 and the immunoglobulin heavy chain gene were identified ; two cases had translocations involving the bcl-1 and the immunoglobulin heavy chain genes .
	manualset3
117729	4	403769	13	NULL	NULL	0	NULL	two cases	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No translocations involving bcl-2 and the immunoglobulin heavy chain gene were identified ; two cases had translocations involving the bcl-1 and the immunoglobulin heavy chain genes .
	manualset3
117730	5	403769	13	NULL	NULL	0	NULL	translocations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	No translocations involving bcl-2 and the immunoglobulin heavy chain gene were identified ; two cases had translocations involving the bcl-1 and the immunoglobulin heavy chain genes .
	manualset3
117731	6	403769	13	NULL	NULL	0	NULL	bcl-1 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	No translocations involving bcl-2 and the immunoglobulin heavy chain gene were identified ; two cases had translocations involving the bcl-1 and the immunoglobulin heavy chain genes .
	manualset3
117732	7	403769	13	NULL	NULL	NULL	NULL	immunoglobulin heavy chain genes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	No translocations involving bcl-2 and the immunoglobulin heavy chain gene were identified ; two cases had translocations involving the bcl-1 and the immunoglobulin heavy chain genes .
	manualset3
117733	1	403770	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	No treatment had been given to 23 patients , 50 had received chemotherapy alone , 23 chemo - and radiotherapy and 14 underwent bone marrow transplantation .
	manualset3
117734	2	403770	13	NULL	NULL	0	NULL	23 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No treatment had been given to 23 patients , 50 had received chemotherapy alone , 23 chemo - and radiotherapy and 14 underwent bone marrow transplantation .
	manualset3
117735	3	403770	13	NULL	NULL	0	NULL	50 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No treatment had been given to 23 patients , 50 had received chemotherapy alone , 23 chemo - and radiotherapy and 14 underwent bone marrow transplantation .
	manualset3
117736	4	403770	13	NULL	NULL	0	NULL	chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	No treatment had been given to 23 patients , 50 had received chemotherapy alone , 23 chemo - and radiotherapy and 14 underwent bone marrow transplantation .
	manualset3
117737	5	403770	13	NULL	NULL	0	NULL	23 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No treatment had been given to 23 patients , 50 had received chemotherapy alone , 23 chemo - and radiotherapy and 14 underwent bone marrow transplantation .
	manualset3
117738	6	403770	13	NULL	NULL	0	NULL	chemotherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	No treatment had been given to 23 patients , 50 had received chemotherapy alone , 23 chemo - and radiotherapy and 14 underwent bone marrow transplantation .
	manualset3
117739	7	403770	13	NULL	NULL	0	NULL	radiotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	No treatment had been given to 23 patients , 50 had received chemotherapy alone , 23 chemo - and radiotherapy and 14 underwent bone marrow transplantation .
	manualset3
117740	8	403770	13	NULL	NULL	0	NULL	 14	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No treatment had been given to 23 patients , 50 had received chemotherapy alone , 23 chemo - and radiotherapy and 14 underwent bone marrow transplantation .
	manualset3
117741	9	403770	13	NULL	NULL	0	NULL	bone marrow transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	No treatment had been given to 23 patients , 50 had received chemotherapy alone , 23 chemo - and radiotherapy and 14 underwent bone marrow transplantation .
	manualset3
117742	1	403771	13	NULL	NULL	0	NULL	AMA-Fab 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	No uptake of AMA-Fab was seen in the regions of previous old infarcts .
	manualset3
117743	2	403771	13	NULL	NULL	0	NULL	regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	No uptake of AMA-Fab was seen in the regions of previous old infarcts .
	manualset3
117744	3	403771	13	NULL	NULL	0	NULL	old infarcts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	No uptake of AMA-Fab was seen in the regions of previous old infarcts .
	manualset3
117745	1	403772	13	NULL	NULL	0	NULL	aneuploidy assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	No well-validated in vitro aneuploidy assay exists , and much research is required to develop tests , perhaps using chromosome counts , DNA content , or effects on cell organelles necessary for mitosis .
	manualset3
117746	2	403772	13	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	No well-validated in vitro aneuploidy assay exists , and much research is required to develop tests , perhaps using chromosome counts , DNA content , or effects on cell organelles necessary for mitosis .
	manualset3
117747	3	403772	13	NULL	NULL	0	NULL	tests	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	No well-validated in vitro aneuploidy assay exists , and much research is required to develop tests , perhaps using chromosome counts , DNA content , or effects on cell organelles necessary for mitosis .
	manualset3
117748	4	403772	13	NULL	NULL	0	NULL	chromosome counts	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No well-validated in vitro aneuploidy assay exists , and much research is required to develop tests , perhaps using chromosome counts , DNA content , or effects on cell organelles necessary for mitosis .
	manualset3
117749	5	403772	13	NULL	NULL	0	NULL	DNA content	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No well-validated in vitro aneuploidy assay exists , and much research is required to develop tests , perhaps using chromosome counts , DNA content , or effects on cell organelles necessary for mitosis .
	manualset3
117750	6	403772	13	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No well-validated in vitro aneuploidy assay exists , and much research is required to develop tests , perhaps using chromosome counts , DNA content , or effects on cell organelles necessary for mitosis .
	manualset3
117751	7	403772	13	NULL	NULL	0	NULL	cell organelles 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	No well-validated in vitro aneuploidy assay exists , and much research is required to develop tests , perhaps using chromosome counts , DNA content , or effects on cell organelles necessary for mitosis .
	manualset3
117752	8	403772	13	NULL	NULL	0	NULL	mitosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	No well-validated in vitro aneuploidy assay exists , and much research is required to develop tests , perhaps using chromosome counts , DNA content , or effects on cell organelles necessary for mitosis .
	manualset3
117753	1	403773	13	NULL	NULL	0	NULL	Nomenclatural changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nomenclatural changes in Phthiraptera - some suggestions .
	manualset3
117754	2	403773	13	NULL	NULL	0	NULL	Phthiraptera 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Nomenclatural changes in Phthiraptera - some suggestions .
	manualset3
117755	3	403773	13	NULL	NULL	0	NULL	suggestions 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nomenclatural changes in Phthiraptera - some suggestions .
	manualset3
117756	1	403774	13	NULL	NULL	NULL	NULL	Nomifensine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nomifensine , benztropine , PCP and amphetamine also inhibited the displacement of ( 3H ) dopamine by ( 1H ) dopamine at concentrations which have been shown previously to inhibit the uptake of ( 3H ) dopamine , suggesting that the mechanism behind displacement and uptake are very similar .
	manualset3
117757	2	403774	13	NULL	NULL	NULL	NULL	benztropine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nomifensine , benztropine , PCP and amphetamine also inhibited the displacement of ( 3H ) dopamine by ( 1H ) dopamine at concentrations which have been shown previously to inhibit the uptake of ( 3H ) dopamine , suggesting that the mechanism behind displacement and uptake are very similar .
	manualset3
117758	3	403774	13	NULL	NULL	NULL	NULL	PCP	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nomifensine , benztropine , PCP and amphetamine also inhibited the displacement of ( 3H ) dopamine by ( 1H ) dopamine at concentrations which have been shown previously to inhibit the uptake of ( 3H ) dopamine , suggesting that the mechanism behind displacement and uptake are very similar .
	manualset3
117759	4	403774	13	NULL	NULL	NULL	NULL	amphetamine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nomifensine , benztropine , PCP and amphetamine also inhibited the displacement of ( 3H ) dopamine by ( 1H ) dopamine at concentrations which have been shown previously to inhibit the uptake of ( 3H ) dopamine , suggesting that the mechanism behind displacement and uptake are very similar .
	manualset3
117760	5	403774	13	NULL	NULL	0	NULL	displacement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nomifensine , benztropine , PCP and amphetamine also inhibited the displacement of ( 3H ) dopamine by ( 1H ) dopamine at concentrations which have been shown previously to inhibit the uptake of ( 3H ) dopamine , suggesting that the mechanism behind displacement and uptake are very similar .
	manualset3
117761	6	403774	13	NULL	NULL	0	NULL	( 3H ) dopamine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nomifensine , benztropine , PCP and amphetamine also inhibited the displacement of ( 3H ) dopamine by ( 1H ) dopamine at concentrations which have been shown previously to inhibit the uptake of ( 3H ) dopamine , suggesting that the mechanism behind displacement and uptake are very similar .
	manualset3
117762	7	403774	13	NULL	NULL	0	NULL	( 1H ) dopamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nomifensine , benztropine , PCP and amphetamine also inhibited the displacement of ( 3H ) dopamine by ( 1H ) dopamine at concentrations which have been shown previously to inhibit the uptake of ( 3H ) dopamine , suggesting that the mechanism behind displacement and uptake are very similar .
	manualset3
117763	8	403774	13	NULL	NULL	0	NULL	concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Nomifensine , benztropine , PCP and amphetamine also inhibited the displacement of ( 3H ) dopamine by ( 1H ) dopamine at concentrations which have been shown previously to inhibit the uptake of ( 3H ) dopamine , suggesting that the mechanism behind displacement and uptake are very similar .
	manualset3
117764	9	403774	13	NULL	NULL	0	NULL	uptake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nomifensine , benztropine , PCP and amphetamine also inhibited the displacement of ( 3H ) dopamine by ( 1H ) dopamine at concentrations which have been shown previously to inhibit the uptake of ( 3H ) dopamine , suggesting that the mechanism behind displacement and uptake are very similar .
	manualset3
117765	10	403774	13	NULL	NULL	0	NULL	( 3H ) dopamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nomifensine , benztropine , PCP and amphetamine also inhibited the displacement of ( 3H ) dopamine by ( 1H ) dopamine at concentrations which have been shown previously to inhibit the uptake of ( 3H ) dopamine , suggesting that the mechanism behind displacement and uptake are very similar .
	manualset3
117766	11	403774	13	NULL	NULL	0	NULL	mechanism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nomifensine , benztropine , PCP and amphetamine also inhibited the displacement of ( 3H ) dopamine by ( 1H ) dopamine at concentrations which have been shown previously to inhibit the uptake of ( 3H ) dopamine , suggesting that the mechanism behind displacement and uptake are very similar .
	manualset3
117767	12	403774	13	NULL	NULL	0	NULL	displacement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nomifensine , benztropine , PCP and amphetamine also inhibited the displacement of ( 3H ) dopamine by ( 1H ) dopamine at concentrations which have been shown previously to inhibit the uptake of ( 3H ) dopamine , suggesting that the mechanism behind displacement and uptake are very similar .
	manualset3
117768	13	403774	13	NULL	NULL	0	NULL	uptake 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nomifensine , benztropine , PCP and amphetamine also inhibited the displacement of ( 3H ) dopamine by ( 1H ) dopamine at concentrations which have been shown previously to inhibit the uptake of ( 3H ) dopamine , suggesting that the mechanism behind displacement and uptake are very similar .
	manualset3
117769	1	403775	13	NULL	NULL	0	NULL	Non-disulphide bridged cysteines 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-disulphide bridged cysteines ( free cysteines ) have no preference for upstream or downstream neighbors .
	manualset3
117770	2	403775	13	NULL	NULL	0	NULL	free cysteines	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-disulphide bridged cysteines ( free cysteines ) have no preference for upstream or downstream neighbors .
	manualset3
117771	3	403775	13	NULL	NULL	0	NULL	upstream neighbors	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-disulphide bridged cysteines ( free cysteines ) have no preference for upstream or downstream neighbors .
	manualset3
117772	4	403775	13	NULL	NULL	0	NULL	downstream neighbors	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-disulphide bridged cysteines ( free cysteines ) have no preference for upstream or downstream neighbors .
	manualset3
117773	1	403776	13	NULL	NULL	0	NULL	induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-hypoxic induction of HIF-3alpha by 2-deoxy-D-glucose and insulin .
	manualset3
117774	2	403776	13	NULL	NULL	0	NULL	HIF-3alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-hypoxic induction of HIF-3alpha by 2-deoxy-D-glucose and insulin .
	manualset3
117775	3	403776	13	NULL	NULL	0	NULL	2-deoxy-D-glucose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-hypoxic induction of HIF-3alpha by 2-deoxy-D-glucose and insulin .
	manualset3
117776	4	403776	13	NULL	NULL	0	NULL	insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-hypoxic induction of HIF-3alpha by 2-deoxy-D-glucose and insulin .
	manualset3
117777	1	403777	13	NULL	NULL	0	NULL	Non-immune ( E ) rosettes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-immune ( E ) rosettes and electrophoretic mobility of peripheral blood lymphocytes of thyroid cancer patients .
	manualset3
117778	2	403777	13	NULL	NULL	0	NULL	electrophoretic mobility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-immune ( E ) rosettes and electrophoretic mobility of peripheral blood lymphocytes of thyroid cancer patients .
	manualset3
117779	3	403777	13	NULL	NULL	0	NULL	 peripheral blood lymphocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-immune ( E ) rosettes and electrophoretic mobility of peripheral blood lymphocytes of thyroid cancer patients .
	manualset3
117780	4	403777	13	NULL	NULL	0	NULL	thyroid cancer patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-immune ( E ) rosettes and electrophoretic mobility of peripheral blood lymphocytes of thyroid cancer patients .
	manualset3
117781	1	403778	13	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-invasive liver iron quantification by SQUID-biosusceptometry and serum ferritin iron as new diagnostic parameters in hereditary hemochromatosis .
	manualset3
117782	2	403778	13	NULL	NULL	0	NULL	iron quantification 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-invasive liver iron quantification by SQUID-biosusceptometry and serum ferritin iron as new diagnostic parameters in hereditary hemochromatosis .
	manualset3
117783	3	403778	13	NULL	NULL	0	NULL	SQUID-biosusceptometry	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-invasive liver iron quantification by SQUID-biosusceptometry and serum ferritin iron as new diagnostic parameters in hereditary hemochromatosis .
	manualset3
117784	4	403778	13	NULL	NULL	0	NULL	serum ferritin iron	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-invasive liver iron quantification by SQUID-biosusceptometry and serum ferritin iron as new diagnostic parameters in hereditary hemochromatosis .
	manualset3
117785	5	403778	13	NULL	NULL	0	NULL	diagnostic parameters	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-invasive liver iron quantification by SQUID-biosusceptometry and serum ferritin iron as new diagnostic parameters in hereditary hemochromatosis .
	manualset3
117786	6	403778	13	NULL	NULL	0	NULL	hereditary hemochromatosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-invasive liver iron quantification by SQUID-biosusceptometry and serum ferritin iron as new diagnostic parameters in hereditary hemochromatosis .
	manualset3
117787	1	403779	13	NULL	NULL	0	NULL	Non-invasive ventilation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-invasive ventilation in amyotrophic lateral sclerosis : a 10 year population based study .
	manualset3
117788	2	403779	13	NULL	NULL	0	NULL	amyotrophic lateral sclerosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-invasive ventilation in amyotrophic lateral sclerosis : a 10 year population based study .
	manualset3
117789	3	403779	13	NULL	NULL	0	NULL	10 year	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-invasive ventilation in amyotrophic lateral sclerosis : a 10 year population based study .
	manualset3
117790	4	403779	13	NULL	NULL	0	NULL	population based study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-invasive ventilation in amyotrophic lateral sclerosis : a 10 year population based study .
	manualset3
117791	1	403780	13	NULL	NULL	0	NULL	Non-necrotizing heparin-induced skin lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-necrotizing heparin-induced skin lesions and the 4T 's score .
	manualset3
117792	2	403780	13	NULL	NULL	0	NULL	4T 's score	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-necrotizing heparin-induced skin lesions and the 4T 's score .
	manualset3
117793	1	403781	13	NULL	NULL	0	NULL	Non-nucleoside reverse transcriptase inhibitors 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-nucleoside reverse transcriptase inhibitors can be used in new therapeutic regimens .
	manualset3
117794	2	403781	13	NULL	NULL	0	NULL	new therapeutic regimens 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-nucleoside reverse transcriptase inhibitors can be used in new therapeutic regimens .
	manualset3
117795	1	403782	13	NULL	NULL	0	NULL	skin conductance responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-specific skin conductance responses indicated that the suppression task was related to similar levels of increased sympathetic activity for both the PTSD and Pre-Deployed groups , whereas the Combat Equivalent group showed no increased activation during thought suppression .
	manualset3
117796	2	403782	13	NULL	NULL	0	NULL	suppression task	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-specific skin conductance responses indicated that the suppression task was related to similar levels of increased sympathetic activity for both the PTSD and Pre-Deployed groups , whereas the Combat Equivalent group showed no increased activation during thought suppression .
	manualset3
117797	3	403782	13	NULL	NULL	0	NULL	levels 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-specific skin conductance responses indicated that the suppression task was related to similar levels of increased sympathetic activity for both the PTSD and Pre-Deployed groups , whereas the Combat Equivalent group showed no increased activation during thought suppression .
	manualset3
117798	4	403782	13	NULL	NULL	0	NULL	sympathetic activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-specific skin conductance responses indicated that the suppression task was related to similar levels of increased sympathetic activity for both the PTSD and Pre-Deployed groups , whereas the Combat Equivalent group showed no increased activation during thought suppression .
	manualset3
117799	5	403782	13	NULL	NULL	0	NULL	PTSD	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-specific skin conductance responses indicated that the suppression task was related to similar levels of increased sympathetic activity for both the PTSD and Pre-Deployed groups , whereas the Combat Equivalent group showed no increased activation during thought suppression .
	manualset3
117800	6	403782	13	NULL	NULL	0	NULL	Pre-Deployed groups 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-specific skin conductance responses indicated that the suppression task was related to similar levels of increased sympathetic activity for both the PTSD and Pre-Deployed groups , whereas the Combat Equivalent group showed no increased activation during thought suppression .
	manualset3
117801	7	403782	13	NULL	NULL	0	NULL	Combat Equivalent group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-specific skin conductance responses indicated that the suppression task was related to similar levels of increased sympathetic activity for both the PTSD and Pre-Deployed groups , whereas the Combat Equivalent group showed no increased activation during thought suppression .
	manualset3
117802	8	403782	13	NULL	NULL	0	NULL	activation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-specific skin conductance responses indicated that the suppression task was related to similar levels of increased sympathetic activity for both the PTSD and Pre-Deployed groups , whereas the Combat Equivalent group showed no increased activation during thought suppression .
	manualset3
117803	9	403782	13	NULL	NULL	0	NULL	thought suppression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-specific skin conductance responses indicated that the suppression task was related to similar levels of increased sympathetic activity for both the PTSD and Pre-Deployed groups , whereas the Combat Equivalent group showed no increased activation during thought suppression .
	manualset3
117804	1	403783	13	NULL	NULL	0	NULL	Non-steroid anti-inflammatory drug therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-steroid anti-inflammatory drug therapy in various fields -- orthopedics ) .
	manualset3
117805	2	403783	13	NULL	NULL	0	NULL	fields	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-steroid anti-inflammatory drug therapy in various fields -- orthopedics ) .
	manualset3
117806	3	403783	13	NULL	NULL	0	NULL	orthopedics	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-steroid anti-inflammatory drug therapy in various fields -- orthopedics ) .
	manualset3
117807	1	403784	13	NULL	NULL	0	NULL	Non-steroidal anti-inflammatory agent	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-steroidal anti-inflammatory agent ibuprofen-induced apoptosis , cell necrosis and cell cycle alterations in human leukemic cells in vitro .
	manualset3
117808	2	403784	13	NULL	NULL	0	NULL	ibuprofen-induced apoptosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-steroidal anti-inflammatory agent ibuprofen-induced apoptosis , cell necrosis and cell cycle alterations in human leukemic cells in vitro .
	manualset3
117809	3	403784	13	NULL	NULL	0	NULL	cell necrosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-steroidal anti-inflammatory agent ibuprofen-induced apoptosis , cell necrosis and cell cycle alterations in human leukemic cells in vitro .
	manualset3
117810	4	403784	13	NULL	NULL	0	NULL	cell cycle alterations 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-steroidal anti-inflammatory agent ibuprofen-induced apoptosis , cell necrosis and cell cycle alterations in human leukemic cells in vitro .
	manualset3
117811	5	403784	13	NULL	NULL	0	NULL	human leukemic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-steroidal anti-inflammatory agent ibuprofen-induced apoptosis , cell necrosis and cell cycle alterations in human leukemic cells in vitro .
	manualset3
117812	1	403785	13	NULL	NULL	0	NULL	Non-urban GPs	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-urban GPs were also significantly more likely to feel less confident in their ability to explain to their patients what to do and why during an influenza pandemic than GPs based in urban areas ( OR 4.68 , 95 % CI 1.78-12 .31 ) .
	manualset3
117813	2	403785	13	NULL	NULL	0	NULL	ability	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-urban GPs were also significantly more likely to feel less confident in their ability to explain to their patients what to do and why during an influenza pandemic than GPs based in urban areas ( OR 4.68 , 95 % CI 1.78-12 .31 ) .
	manualset3
117814	3	403785	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-urban GPs were also significantly more likely to feel less confident in their ability to explain to their patients what to do and why during an influenza pandemic than GPs based in urban areas ( OR 4.68 , 95 % CI 1.78-12 .31 ) .
	manualset3
117815	4	403785	13	NULL	NULL	0	NULL	influenza pandemic	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-urban GPs were also significantly more likely to feel less confident in their ability to explain to their patients what to do and why during an influenza pandemic than GPs based in urban areas ( OR 4.68 , 95 % CI 1.78-12 .31 ) .
	manualset3
117816	5	403785	13	NULL	NULL	0	NULL	GPs 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-urban GPs were also significantly more likely to feel less confident in their ability to explain to their patients what to do and why during an influenza pandemic than GPs based in urban areas ( OR 4.68 , 95 % CI 1.78-12 .31 ) .
	manualset3
117817	6	403785	13	NULL	NULL	0	NULL	urban areas 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-urban GPs were also significantly more likely to feel less confident in their ability to explain to their patients what to do and why during an influenza pandemic than GPs based in urban areas ( OR 4.68 , 95 % CI 1.78-12 .31 ) .
	manualset3
117818	7	403785	13	NULL	NULL	0	NULL	OR 4.68 , 95 % CI 1.78-12 .31 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Non-urban GPs were also significantly more likely to feel less confident in their ability to explain to their patients what to do and why during an influenza pandemic than GPs based in urban areas ( OR 4.68 , 95 % CI 1.78-12 .31 ) .
	manualset3
117819	1	403786	13	NULL	NULL	0	NULL	Nonablative skin remodeling 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonablative skin remodeling has become an attractive option for patients whose lifestyles demand a noninvasive approach to skin rejuvenation .
	manualset3
117820	2	403786	13	NULL	NULL	0	NULL	attractive option 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonablative skin remodeling has become an attractive option for patients whose lifestyles demand a noninvasive approach to skin rejuvenation .
	manualset3
117821	3	403786	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonablative skin remodeling has become an attractive option for patients whose lifestyles demand a noninvasive approach to skin rejuvenation .
	manualset3
117822	4	403786	13	NULL	NULL	0	NULL	lifestyles	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonablative skin remodeling has become an attractive option for patients whose lifestyles demand a noninvasive approach to skin rejuvenation .
	manualset3
117823	5	403786	13	NULL	NULL	0	NULL	noninvasive approach	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonablative skin remodeling has become an attractive option for patients whose lifestyles demand a noninvasive approach to skin rejuvenation .
	manualset3
117824	6	403786	13	NULL	NULL	0	NULL	skin rejuvenation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonablative skin remodeling has become an attractive option for patients whose lifestyles demand a noninvasive approach to skin rejuvenation .
	manualset3
117825	1	403787	13	NULL	NULL	0	NULL	Nonadrenergic , noncholinergic ( NANC ) contraction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonadrenergic , noncholinergic ( NANC ) contraction has been demonstrated in animal urinary bladder .
	manualset3
117826	2	403787	13	NULL	NULL	0	NULL	animal urinary bladder	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonadrenergic , noncholinergic ( NANC ) contraction has been demonstrated in animal urinary bladder .
	manualset3
117827	1	403788	13	NULL	NULL	0	NULL	computerized tomography ( CT ) scan	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A computerized tomography ( CT ) scan of the abdomen showed cirrhotic liver , evidence of esophageal varices , but no evidence of a liver mass. .
	manualset3
117828	2	403788	13	NULL	NULL	0	NULL	abdomen 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A computerized tomography ( CT ) scan of the abdomen showed cirrhotic liver , evidence of esophageal varices , but no evidence of a liver mass. .
	manualset3
117829	3	403788	13	NULL	NULL	0	NULL	cirrhotic liver	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A computerized tomography ( CT ) scan of the abdomen showed cirrhotic liver , evidence of esophageal varices , but no evidence of a liver mass. .
	manualset3
117830	4	403788	13	NULL	NULL	0	NULL	evidence of esophageal varices	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A computerized tomography ( CT ) scan of the abdomen showed cirrhotic liver , evidence of esophageal varices , but no evidence of a liver mass. .
	manualset3
117831	5	403788	13	NULL	NULL	0	NULL	evidence of a liver mass	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A computerized tomography ( CT ) scan of the abdomen showed cirrhotic liver , evidence of esophageal varices , but no evidence of a liver mass. .
	manualset3
117832	1	403789	13	NULL	NULL	0	NULL	Nonaromatic products 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonaromatic products from anoxic conversion of benzoyl-CoA with benzoyl-CoA reductase and cyclohexa-1 , 5 - diene-1-carbonyl-CoA hydratase .
	manualset3
117833	2	403789	13	NULL	NULL	0	NULL	anoxic conversion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonaromatic products from anoxic conversion of benzoyl-CoA with benzoyl-CoA reductase and cyclohexa-1 , 5 - diene-1-carbonyl-CoA hydratase .
	manualset3
117834	3	403789	13	NULL	NULL	0	NULL	benzoyl-CoA 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonaromatic products from anoxic conversion of benzoyl-CoA with benzoyl-CoA reductase and cyclohexa-1 , 5 - diene-1-carbonyl-CoA hydratase .
	manualset3
117835	4	403789	13	NULL	NULL	0	NULL	benzoyl-CoA reductase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonaromatic products from anoxic conversion of benzoyl-CoA with benzoyl-CoA reductase and cyclohexa-1 , 5 - diene-1-carbonyl-CoA hydratase .
	manualset3
117836	5	403789	13	NULL	NULL	0	NULL	cyclohexa-1 , 5 - diene-1-carbonyl-CoA hydratase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonaromatic products from anoxic conversion of benzoyl-CoA with benzoyl-CoA reductase and cyclohexa-1 , 5 - diene-1-carbonyl-CoA hydratase .
	manualset3
117837	1	403790	13	NULL	NULL	0	NULL	Noncompliance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Noncompliance in community psychiatry : a review of clinical interventions .
	manualset3
117838	2	403790	13	NULL	NULL	0	NULL	community psychiatry 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Noncompliance in community psychiatry : a review of clinical interventions .
	manualset3
117839	3	403790	13	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Noncompliance in community psychiatry : a review of clinical interventions .
	manualset3
117840	4	403790	13	NULL	NULL	0	NULL	clinical interventions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Noncompliance in community psychiatry : a review of clinical interventions .
	manualset3
117841	1	403791	13	NULL	NULL	0	NULL	10 % dip	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Nondipping was defined as less than a 10 % dip in sleep BP compared with wake BP .
	manualset3
117842	2	403791	13	NULL	NULL	0	NULL	sleep BP	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nondipping was defined as less than a 10 % dip in sleep BP compared with wake BP .
	manualset3
117843	3	403791	13	NULL	NULL	0	NULL	wake BP	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nondipping was defined as less than a 10 % dip in sleep BP compared with wake BP .
	manualset3
117844	1	403792	13	NULL	NULL	0	NULL	VP1-immunized mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the VP1-immunized mice developed diabetes , irrespective of the interval between immunization and virus challenge , whereas 80 to 95 % of the EMC-D virus-infected control mice did develop diabetes .
	manualset3
117845	2	403792	13	NULL	NULL	0	NULL	diabetes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the VP1-immunized mice developed diabetes , irrespective of the interval between immunization and virus challenge , whereas 80 to 95 % of the EMC-D virus-infected control mice did develop diabetes .
	manualset3
117846	3	403792	13	NULL	NULL	0	NULL	interval	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the VP1-immunized mice developed diabetes , irrespective of the interval between immunization and virus challenge , whereas 80 to 95 % of the EMC-D virus-infected control mice did develop diabetes .
	manualset3
117847	4	403792	13	NULL	NULL	0	NULL	immunization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the VP1-immunized mice developed diabetes , irrespective of the interval between immunization and virus challenge , whereas 80 to 95 % of the EMC-D virus-infected control mice did develop diabetes .
	manualset3
117848	5	403792	13	NULL	NULL	0	NULL	virus challenge	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the VP1-immunized mice developed diabetes , irrespective of the interval between immunization and virus challenge , whereas 80 to 95 % of the EMC-D virus-infected control mice did develop diabetes .
	manualset3
117849	6	403792	13	NULL	NULL	0	NULL	80 to 95 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the VP1-immunized mice developed diabetes , irrespective of the interval between immunization and virus challenge , whereas 80 to 95 % of the EMC-D virus-infected control mice did develop diabetes .
	manualset3
117850	7	403792	13	NULL	NULL	0	NULL	EMC-D virus-infected control mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the VP1-immunized mice developed diabetes , irrespective of the interval between immunization and virus challenge , whereas 80 to 95 % of the EMC-D virus-infected control mice did develop diabetes .
	manualset3
117851	8	403792	13	NULL	NULL	0	NULL	diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the VP1-immunized mice developed diabetes , irrespective of the interval between immunization and virus challenge , whereas 80 to 95 % of the EMC-D virus-infected control mice did develop diabetes .
	manualset3
117852	1	403793	13	NULL	NULL	0	NULL	`` C. upsaliensis '' strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the `` C. upsaliensis '' strains could be agglutinated with antisera against heat-labile antigens from C. jejuni , C. coli , or C. laridis .
	manualset3
117853	2	403793	13	NULL	NULL	0	NULL	antisera	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the `` C. upsaliensis '' strains could be agglutinated with antisera against heat-labile antigens from C. jejuni , C. coli , or C. laridis .
	manualset3
117854	3	403793	13	NULL	NULL	0	NULL	heat-labile antigens 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the `` C. upsaliensis '' strains could be agglutinated with antisera against heat-labile antigens from C. jejuni , C. coli , or C. laridis .
	manualset3
117855	4	403793	13	NULL	NULL	0	NULL	C. jejuni	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the `` C. upsaliensis '' strains could be agglutinated with antisera against heat-labile antigens from C. jejuni , C. coli , or C. laridis .
	manualset3
117856	5	403793	13	NULL	NULL	0	NULL	C. coli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the `` C. upsaliensis '' strains could be agglutinated with antisera against heat-labile antigens from C. jejuni , C. coli , or C. laridis .
	manualset3
117857	6	403793	13	NULL	NULL	0	NULL	C. laridis 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the `` C. upsaliensis '' strains could be agglutinated with antisera against heat-labile antigens from C. jejuni , C. coli , or C. laridis .
	manualset3
117858	1	403794	13	NULL	NULL	0	NULL	antagonists	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the antagonists used had any effect on basal PRL secretion .
	manualset3
117859	2	403794	13	NULL	NULL	0	NULL	effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the antagonists used had any effect on basal PRL secretion .
	manualset3
117860	3	403794	13	NULL	NULL	0	NULL	basal PRL secretion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the antagonists used had any effect on basal PRL secretion .
	manualset3
117861	1	403795	13	NULL	NULL	0	NULL	compounds 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the compounds tested inhibit the activity of related enzymes ( NPP6 and NPP7 ) .
	manualset3
117862	2	403795	13	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the compounds tested inhibit the activity of related enzymes ( NPP6 and NPP7 ) .
	manualset3
117863	3	403795	13	NULL	NULL	0	NULL	related enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the compounds tested inhibit the activity of related enzymes ( NPP6 and NPP7 ) .
	manualset3
117864	4	403795	13	NULL	NULL	0	NULL	NPP6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the compounds tested inhibit the activity of related enzymes ( NPP6 and NPP7 ) .
	manualset3
117865	5	403795	13	NULL	NULL	0	NULL	NPP7	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the compounds tested inhibit the activity of related enzymes ( NPP6 and NPP7 ) .
	manualset3
117866	1	403796	13	NULL	NULL	0	NULL	decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A concomitant decrease in albumin and urea synthesis was also observed .
	manualset3
117867	2	403796	13	NULL	NULL	0	NULL	albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A concomitant decrease in albumin and urea synthesis was also observed .
	manualset3
117868	3	403796	13	NULL	NULL	0	NULL	urea synthesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A concomitant decrease in albumin and urea synthesis was also observed .
	manualset3
117869	1	403797	13	NULL	NULL	0	NULL	factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the factors that have been found to be associated with osteonecrosis in patients with systemic lupus erythematosus could be associated with disease progression .
	manualset3
117870	2	403797	13	NULL	NULL	0	NULL	osteonecrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the factors that have been found to be associated with osteonecrosis in patients with systemic lupus erythematosus could be associated with disease progression .
	manualset3
117871	3	403797	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the factors that have been found to be associated with osteonecrosis in patients with systemic lupus erythematosus could be associated with disease progression .
	manualset3
117873	4	403797	13	NULL	NULL	NULL	NULL	 systemic lupus erythematosus 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	None of the factors that have been found to be associated with osteonecrosis in patients with systemic lupus erythematosus could be associated with disease progression .
	manualset3
117874	5	403797	13	NULL	NULL	0	NULL	disease progression 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the factors that have been found to be associated with osteonecrosis in patients with systemic lupus erythematosus could be associated with disease progression .
	manualset3
117875	1	403798	13	NULL	NULL	0	NULL	new-generation bonding systems	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the new-generation bonding systems was significantly more effective in reducing microleakage than Light Cured Scotchbond .
	manualset3
117876	2	403798	13	NULL	NULL	0	NULL	microleakage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the new-generation bonding systems was significantly more effective in reducing microleakage than Light Cured Scotchbond .
	manualset3
117877	3	403798	13	NULL	NULL	0	NULL	Light Cured Scotchbond	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the new-generation bonding systems was significantly more effective in reducing microleakage than Light Cured Scotchbond .
	manualset3
117878	1	403799	13	NULL	NULL	0	NULL	pFSH-PVP treatments 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the pFSH-PVP treatments were effective in inducing superovulation .
	manualset3
117879	2	403799	13	NULL	NULL	0	NULL	superovulation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the pFSH-PVP treatments were effective in inducing superovulation .
	manualset3
117880	1	403800	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the patients had the G to C mutation at the same position .
	manualset3
117881	2	403800	13	NULL	NULL	0	NULL	G to C mutation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the patients had the G to C mutation at the same position .
	manualset3
117882	3	403800	13	NULL	NULL	NULL	NULL	position	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	None of the patients had the G to C mutation at the same position .
	manualset3
117883	1	403801	13	NULL	NULL	0	NULL	restorative materials	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the restorative materials evaluated affected the growth of L casei , S sobrinus , or S mutans at all time periods including baseline , where fluoride was detected in the agar beneath the specimen disks .
	manualset3
117884	2	403801	13	NULL	NULL	0	NULL	growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the restorative materials evaluated affected the growth of L casei , S sobrinus , or S mutans at all time periods including baseline , where fluoride was detected in the agar beneath the specimen disks .
	manualset3
117885	3	403801	13	NULL	NULL	0	NULL	L casei 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the restorative materials evaluated affected the growth of L casei , S sobrinus , or S mutans at all time periods including baseline , where fluoride was detected in the agar beneath the specimen disks .
	manualset3
117886	4	403801	13	NULL	NULL	0	NULL	S sobrinus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the restorative materials evaluated affected the growth of L casei , S sobrinus , or S mutans at all time periods including baseline , where fluoride was detected in the agar beneath the specimen disks .
	manualset3
117887	5	403801	13	NULL	NULL	0	NULL	S mutan	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the restorative materials evaluated affected the growth of L casei , S sobrinus , or S mutans at all time periods including baseline , where fluoride was detected in the agar beneath the specimen disks .
	manualset3
117888	6	403801	13	NULL	NULL	0	NULL	time periods	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the restorative materials evaluated affected the growth of L casei , S sobrinus , or S mutans at all time periods including baseline , where fluoride was detected in the agar beneath the specimen disks .
	manualset3
117889	7	403801	13	NULL	NULL	0	NULL	baseline	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the restorative materials evaluated affected the growth of L casei , S sobrinus , or S mutans at all time periods including baseline , where fluoride was detected in the agar beneath the specimen disks .
	manualset3
117890	8	403801	13	NULL	NULL	0	NULL	fluoride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the restorative materials evaluated affected the growth of L casei , S sobrinus , or S mutans at all time periods including baseline , where fluoride was detected in the agar beneath the specimen disks .
	manualset3
117891	9	403801	13	NULL	NULL	0	NULL	agar	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the restorative materials evaluated affected the growth of L casei , S sobrinus , or S mutans at all time periods including baseline , where fluoride was detected in the agar beneath the specimen disks .
	manualset3
117892	10	403801	13	NULL	NULL	0	NULL	specimen disks	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	None of the restorative materials evaluated affected the growth of L casei , S sobrinus , or S mutans at all time periods including baseline , where fluoride was detected in the agar beneath the specimen disks .
	manualset3
117893	1	403802	13	NULL	NULL	0	NULL	changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	None of these changes was seen in control macrophages or those exposed to recombinant interferon-gamma ( IFN ) .
	manualset3
117894	2	403802	13	NULL	NULL	0	NULL	control macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	None of these changes was seen in control macrophages or those exposed to recombinant interferon-gamma ( IFN ) .
	manualset3
117895	3	403802	13	NULL	NULL	0	NULL	recombinant interferon-gamma ( IFN )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	None of these changes was seen in control macrophages or those exposed to recombinant interferon-gamma ( IFN ) .
	manualset3
117896	1	403803	13	NULL	NULL	0	NULL	conditioned stimulus ( CS ) exposure	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A conditioned stimulus ( CS ) exposure has the ability to induce two qualitatively different mnesic processes : memory reconsolidation and memory extinction .
	manualset3
117897	2	403803	13	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A conditioned stimulus ( CS ) exposure has the ability to induce two qualitatively different mnesic processes : memory reconsolidation and memory extinction .
	manualset3
117898	3	403803	13	NULL	NULL	0	NULL	mnesic processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A conditioned stimulus ( CS ) exposure has the ability to induce two qualitatively different mnesic processes : memory reconsolidation and memory extinction .
	manualset3
117899	4	403803	13	NULL	NULL	0	NULL	memory reconsolidation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A conditioned stimulus ( CS ) exposure has the ability to induce two qualitatively different mnesic processes : memory reconsolidation and memory extinction .
	manualset3
117900	5	403803	13	NULL	NULL	0	NULL	memory extinction 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A conditioned stimulus ( CS ) exposure has the ability to induce two qualitatively different mnesic processes : memory reconsolidation and memory extinction .
	manualset3
117901	1	403804	13	NULL	NULL	0	NULL	endogenous compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	None of these endogenous compounds has been shown conclusively to modulate sodium pump activity by binding to the cardiac glycoside binding site on Na + , K + - ATPase .
	manualset3
117902	2	403804	13	NULL	NULL	0	NULL	sodium pump activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	None of these endogenous compounds has been shown conclusively to modulate sodium pump activity by binding to the cardiac glycoside binding site on Na + , K + - ATPase .
	manualset3
117903	3	403804	13	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	None of these endogenous compounds has been shown conclusively to modulate sodium pump activity by binding to the cardiac glycoside binding site on Na + , K + - ATPase .
	manualset3
117904	4	403804	13	NULL	NULL	0	NULL	cardiac glycoside binding site 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	None of these endogenous compounds has been shown conclusively to modulate sodium pump activity by binding to the cardiac glycoside binding site on Na + , K + - ATPase .
	manualset3
117905	5	403804	13	NULL	NULL	0	NULL	Na + , K + - ATPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	None of these endogenous compounds has been shown conclusively to modulate sodium pump activity by binding to the cardiac glycoside binding site on Na + , K + - ATPase .
	manualset3
117906	1	403805	13	NULL	NULL	0	NULL	measures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	None of these measures indicated a difference in hydration status as a result of the dietary intervention in either the control or tea condition .
	manualset3
117907	2	403805	13	NULL	NULL	0	NULL	difference 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	None of these measures indicated a difference in hydration status as a result of the dietary intervention in either the control or tea condition .
	manualset3
117908	3	403805	13	NULL	NULL	0	NULL	hydration status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	None of these measures indicated a difference in hydration status as a result of the dietary intervention in either the control or tea condition .
	manualset3
117909	4	403805	13	NULL	NULL	0	NULL	result	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	None of these measures indicated a difference in hydration status as a result of the dietary intervention in either the control or tea condition .
	manualset3
117910	5	403805	13	NULL	NULL	0	NULL	dietary intervention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	None of these measures indicated a difference in hydration status as a result of the dietary intervention in either the control or tea condition .
	manualset3
117911	6	403805	13	NULL	NULL	0	NULL	control	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	None of these measures indicated a difference in hydration status as a result of the dietary intervention in either the control or tea condition .
	manualset3
117912	7	403805	13	NULL	NULL	0	NULL	tea condition	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	None of these measures indicated a difference in hydration status as a result of the dietary intervention in either the control or tea condition .
	manualset3
117913	1	403806	13	NULL	NULL	0	NULL	damage 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	None showed primary damage to type 2 pneumocytes .
	manualset3
117914	2	403806	13	NULL	NULL	0	NULL	type 2 pneumocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	None showed primary damage to type 2 pneumocytes .
	manualset3
117915	1	403807	13	NULL	NULL	0	NULL	Nonenzymatic anticoagulant activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonenzymatic anticoagulant activity of the mutant serine protease Ser360Ala-activated protein C mediated by factor Va .
	manualset3
117916	2	403807	13	NULL	NULL	0	NULL	mutant serine protease Ser360Ala-activated protein C 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonenzymatic anticoagulant activity of the mutant serine protease Ser360Ala-activated protein C mediated by factor Va .
	manualset3
117917	3	403807	13	NULL	NULL	0	NULL	factor Va	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonenzymatic anticoagulant activity of the mutant serine protease Ser360Ala-activated protein C mediated by factor Va .
	manualset3
117918	1	403808	13	NULL	NULL	0	NULL	Nonenzymatic hydroxylations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonenzymatic hydroxylations of proline and lysine by reduced oxygen derivatives .
	manualset3
117919	2	403808	13	NULL	NULL	0	NULL	proline	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonenzymatic hydroxylations of proline and lysine by reduced oxygen derivatives .
	manualset3
117920	3	403808	13	NULL	NULL	0	NULL	lysine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonenzymatic hydroxylations of proline and lysine by reduced oxygen derivatives .
	manualset3
117921	4	403808	13	NULL	NULL	0	NULL	reduced oxygen derivatives	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonenzymatic hydroxylations of proline and lysine by reduced oxygen derivatives .
	manualset3
117922	1	403809	13	NULL	NULL	0	NULL	Nonessential activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonessential activation and competitive inhibition of bacterial phosphatidylinositol-specific phospholipase C by short-chain phospholipids and analogs .
	manualset3
117923	2	403809	13	NULL	NULL	0	NULL	competitive inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonessential activation and competitive inhibition of bacterial phosphatidylinositol-specific phospholipase C by short-chain phospholipids and analogs .
	manualset3
117924	3	403809	13	NULL	NULL	0	NULL	bacterial phosphatidylinositol-specific phospholipase C	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonessential activation and competitive inhibition of bacterial phosphatidylinositol-specific phospholipase C by short-chain phospholipids and analogs .
	manualset3
117925	4	403809	13	NULL	NULL	0	NULL	short-chain phospholipids 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonessential activation and competitive inhibition of bacterial phosphatidylinositol-specific phospholipase C by short-chain phospholipids and analogs .
	manualset3
117926	5	403809	13	NULL	NULL	0	NULL	analogs 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonessential activation and competitive inhibition of bacterial phosphatidylinositol-specific phospholipase C by short-chain phospholipids and analogs .
	manualset3
117927	1	403810	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonetheless , in the patients with far-advanced CRF , IL-10 mRNA levels ( 20 + / -10 ) were lower ( p & lt ; 0.05 ) than in the patients with less-advanced CRF and not significantly different than in the healthy controls .
	manualset3
117928	2	403810	13	NULL	NULL	0	NULL	far-advanced CRF	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonetheless , in the patients with far-advanced CRF , IL-10 mRNA levels ( 20 + / -10 ) were lower ( p & lt ; 0.05 ) than in the patients with less-advanced CRF and not significantly different than in the healthy controls .
	manualset3
117929	3	403810	13	NULL	NULL	0	NULL	IL-10 mRNA levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonetheless , in the patients with far-advanced CRF , IL-10 mRNA levels ( 20 + / -10 ) were lower ( p & lt ; 0.05 ) than in the patients with less-advanced CRF and not significantly different than in the healthy controls .
	manualset3
117930	4	403810	13	NULL	NULL	0	NULL	20 + / -10	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonetheless , in the patients with far-advanced CRF , IL-10 mRNA levels ( 20 + / -10 ) were lower ( p & lt ; 0.05 ) than in the patients with less-advanced CRF and not significantly different than in the healthy controls .
	manualset3
117931	5	403810	13	NULL	NULL	0	NULL	p & lt ; 0.05 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonetheless , in the patients with far-advanced CRF , IL-10 mRNA levels ( 20 + / -10 ) were lower ( p & lt ; 0.05 ) than in the patients with less-advanced CRF and not significantly different than in the healthy controls .
	manualset3
117932	6	403810	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonetheless , in the patients with far-advanced CRF , IL-10 mRNA levels ( 20 + / -10 ) were lower ( p & lt ; 0.05 ) than in the patients with less-advanced CRF and not significantly different than in the healthy controls .
	manualset3
117933	7	403810	13	NULL	NULL	0	NULL	less-advanced CRF	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonetheless , in the patients with far-advanced CRF , IL-10 mRNA levels ( 20 + / -10 ) were lower ( p & lt ; 0.05 ) than in the patients with less-advanced CRF and not significantly different than in the healthy controls .
	manualset3
117934	8	403810	13	NULL	NULL	0	NULL	healthy controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonetheless , in the patients with far-advanced CRF , IL-10 mRNA levels ( 20 + / -10 ) were lower ( p & lt ; 0.05 ) than in the patients with less-advanced CRF and not significantly different than in the healthy controls .
	manualset3
117935	1	403811	13	NULL	NULL	NULL	NULL	Biomechanical investigation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Biomechanical investigation of fixed-angle plate osteosynthesis of the proximal humerus ) .
	manualset3
117936	2	403811	13	NULL	NULL	0	NULL	fixed-angle plate osteosynthesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Biomechanical investigation of fixed-angle plate osteosynthesis of the proximal humerus ) .
	manualset3
117937	3	403811	13	NULL	NULL	0	NULL	proximal humerus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Biomechanical investigation of fixed-angle plate osteosynthesis of the proximal humerus ) .
	manualset3
117938	1	403812	13	NULL	NULL	0	NULL	logistic regression analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonetheless , logistic regression analyses did not provide evidence linking marginal productivity to p , p ' - DDE , total PCBs , or arylhydrocarbon receptor-active PCB congener exposure in regions of concern .
	manualset3
117939	2	403812	13	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonetheless , logistic regression analyses did not provide evidence linking marginal productivity to p , p ' - DDE , total PCBs , or arylhydrocarbon receptor-active PCB congener exposure in regions of concern .
	manualset3
117940	3	403812	13	NULL	NULL	0	NULL	marginal productivity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonetheless , logistic regression analyses did not provide evidence linking marginal productivity to p , p ' - DDE , total PCBs , or arylhydrocarbon receptor-active PCB congener exposure in regions of concern .
	manualset3
117941	4	403812	13	NULL	NULL	0	NULL	p , p ' - DDE 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonetheless , logistic regression analyses did not provide evidence linking marginal productivity to p , p ' - DDE , total PCBs , or arylhydrocarbon receptor-active PCB congener exposure in regions of concern .
	manualset3
117942	5	403812	13	NULL	NULL	0	NULL	total PCBs	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonetheless , logistic regression analyses did not provide evidence linking marginal productivity to p , p ' - DDE , total PCBs , or arylhydrocarbon receptor-active PCB congener exposure in regions of concern .
	manualset3
117943	6	403812	13	NULL	NULL	0	NULL	arylhydrocarbon receptor-active PCB congener 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonetheless , logistic regression analyses did not provide evidence linking marginal productivity to p , p ' - DDE , total PCBs , or arylhydrocarbon receptor-active PCB congener exposure in regions of concern .
	manualset3
117944	7	403812	13	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonetheless , logistic regression analyses did not provide evidence linking marginal productivity to p , p ' - DDE , total PCBs , or arylhydrocarbon receptor-active PCB congener exposure in regions of concern .
	manualset3
117945	8	403812	13	NULL	NULL	0	NULL	regions of concern	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonetheless , logistic regression analyses did not provide evidence linking marginal productivity to p , p ' - DDE , total PCBs , or arylhydrocarbon receptor-active PCB congener exposure in regions of concern .
	manualset3
117946	1	403813	13	NULL	NULL	0	NULL	permanent pores	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonetheless , permanent pores are formed as confirmed by PXRD and gas sorption analysis .
	manualset3
117947	2	403813	13	NULL	NULL	0	NULL	PXRD 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonetheless , permanent pores are formed as confirmed by PXRD and gas sorption analysis .
	manualset3
117948	3	403813	13	NULL	NULL	0	NULL	gas sorption analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonetheless , permanent pores are formed as confirmed by PXRD and gas sorption analysis .
	manualset3
117949	1	403814	13	NULL	NULL	0	NULL	globular domain of the Mre11 complex	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonhomologous end joining , which is probably mediated by the globular domain of the Mre11 complex , was also severely impaired by alteration of the coiled-coil and hook domains , providing the first evidence of their influence on this process .
	manualset3
117950	2	403814	13	NULL	NULL	0	NULL	alteration	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonhomologous end joining , which is probably mediated by the globular domain of the Mre11 complex , was also severely impaired by alteration of the coiled-coil and hook domains , providing the first evidence of their influence on this process .
	manualset3
117951	3	403814	13	NULL	NULL	0	NULL	coiled-coil domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonhomologous end joining , which is probably mediated by the globular domain of the Mre11 complex , was also severely impaired by alteration of the coiled-coil and hook domains , providing the first evidence of their influence on this process .
	manualset3
117952	4	403814	13	NULL	NULL	0	NULL	hook domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonhomologous end joining , which is probably mediated by the globular domain of the Mre11 complex , was also severely impaired by alteration of the coiled-coil and hook domains , providing the first evidence of their influence on this process .
	manualset3
117953	5	403814	13	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonhomologous end joining , which is probably mediated by the globular domain of the Mre11 complex , was also severely impaired by alteration of the coiled-coil and hook domains , providing the first evidence of their influence on this process .
	manualset3
117954	6	403814	13	NULL	NULL	0	NULL	influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonhomologous end joining , which is probably mediated by the globular domain of the Mre11 complex , was also severely impaired by alteration of the coiled-coil and hook domains , providing the first evidence of their influence on this process .
	manualset3
117955	7	403814	13	NULL	NULL	0	NULL	process 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonhomologous end joining , which is probably mediated by the globular domain of the Mre11 complex , was also severely impaired by alteration of the coiled-coil and hook domains , providing the first evidence of their influence on this process .
	manualset3
120447	8	403814	13	NULL	NULL	0	NULL	Nonhomologous end joining	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonhomologous end joining , which is probably mediated by the globular domain of the Mre11 complex , was also severely impaired by alteration of the coiled-coil and hook domains , providing the first evidence of their influence on this process .
	manualset3
117956	1	403815	13	NULL	NULL	0	NULL	Noninfectious causes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Noninfectious causes of immunosuppression in dogs and cats .
	manualset3
117957	2	403815	13	NULL	NULL	0	NULL	immunosuppression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Noninfectious causes of immunosuppression in dogs and cats .
	manualset3
117958	3	403815	13	NULL	NULL	0	NULL	dogs 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Noninfectious causes of immunosuppression in dogs and cats .
	manualset3
117959	4	403815	13	NULL	NULL	0	NULL	cats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Noninfectious causes of immunosuppression in dogs and cats .
	manualset3
117960	1	403816	13	NULL	NULL	0	NULL	Noninvasive coronary angiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Noninvasive coronary angiography by magnetic resonance imaging , electron-beam computed tomography , and multislice computed tomography .
	manualset3
117961	2	403816	13	NULL	NULL	0	NULL	magnetic resonance imaging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Noninvasive coronary angiography by magnetic resonance imaging , electron-beam computed tomography , and multislice computed tomography .
	manualset3
117962	3	403816	13	NULL	NULL	0	NULL	electron-beam computed tomography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Noninvasive coronary angiography by magnetic resonance imaging , electron-beam computed tomography , and multislice computed tomography .
	manualset3
117963	4	403816	13	NULL	NULL	0	NULL	multislice computed tomography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Noninvasive coronary angiography by magnetic resonance imaging , electron-beam computed tomography , and multislice computed tomography .
	manualset3
117964	1	403817	13	NULL	NULL	0	NULL	Noninvasive genetic sampling approaches	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Noninvasive genetic sampling approaches are becoming increasingly important to study wildlife populations .
	manualset3
117965	2	403817	13	NULL	NULL	0	NULL	wildlife populations	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Noninvasive genetic sampling approaches are becoming increasingly important to study wildlife populations .
	manualset3
117966	1	403818	13	NULL	NULL	0	NULL	Nonlethal infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonlethal infection of laboratory mice induced with `` mouse '' rabies strains .
	manualset3
117967	2	403818	13	NULL	NULL	0	NULL	laboratory mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonlethal infection of laboratory mice induced with `` mouse '' rabies strains .
	manualset3
117968	3	403818	13	NULL	NULL	0	NULL	`` mouse '' rabies strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonlethal infection of laboratory mice induced with `` mouse '' rabies strains .
	manualset3
117969	1	403819	13	NULL	NULL	0	NULL	Nonlinear analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonlinear analysis and prediction of coarse particulate matter concentration in ambient air .
	manualset3
117970	2	403819	13	NULL	NULL	0	NULL	prediction 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonlinear analysis and prediction of coarse particulate matter concentration in ambient air .
	manualset3
117971	3	403819	13	NULL	NULL	0	NULL	coarse particulate matter	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonlinear analysis and prediction of coarse particulate matter concentration in ambient air .
	manualset3
117972	4	403819	13	NULL	NULL	0	NULL	concentration 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonlinear analysis and prediction of coarse particulate matter concentration in ambient air .
	manualset3
117973	5	403819	13	NULL	NULL	0	NULL	ambient air	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonlinear analysis and prediction of coarse particulate matter concentration in ambient air .
	manualset3
117974	1	403820	13	NULL	NULL	0	NULL	Nonlinear screening	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonlinear screening and gas-liquid separation in suspensions of charged colloids .
	manualset3
117975	2	403820	13	NULL	NULL	0	NULL	gas-liquid separation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonlinear screening and gas-liquid separation in suspensions of charged colloids .
	manualset3
117976	3	403820	13	NULL	NULL	0	NULL	suspensions of charged colloids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonlinear screening and gas-liquid separation in suspensions of charged colloids .
	manualset3
117977	1	403821	13	NULL	NULL	0	NULL	Nonnatural amino acid ligands	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonnatural amino acid ligands in heme protein design .
	manualset3
117978	2	403821	13	NULL	NULL	0	NULL	heme protein design	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonnatural amino acid ligands in heme protein design .
	manualset3
117979	1	403822	13	NULL	NULL	0	NULL	Nonneoplastic mucocutaneous lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonneoplastic mucocutaneous lesions in organ transplant recipients .
	manualset3
117980	2	403822	13	NULL	NULL	0	NULL	organ transplant recipients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonneoplastic mucocutaneous lesions in organ transplant recipients .
	manualset3
117981	1	403823	13	NULL	NULL	0	NULL	Nonsense mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonsense mutations of both sqt-1 and rol-6 cause nearly , but not totally , wild-type phenotypes .
	manualset3
117982	2	403823	13	NULL	NULL	0	NULL	sqt-1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonsense mutations of both sqt-1 and rol-6 cause nearly , but not totally , wild-type phenotypes .
	manualset3
117983	3	403823	13	NULL	NULL	0	NULL	rol-6	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonsense mutations of both sqt-1 and rol-6 cause nearly , but not totally , wild-type phenotypes .
	manualset3
117984	4	403823	13	NULL	NULL	0	NULL	wild-type phenotypes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonsense mutations of both sqt-1 and rol-6 cause nearly , but not totally , wild-type phenotypes .
	manualset3
117985	1	403824	13	NULL	NULL	0	NULL	Nonsteroidal anti-inflammatory drugs ( NSAIDs )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonsteroidal anti-inflammatory drugs ( NSAIDs ) cause acute diffuse injury to the gastroduodenal mucosa , and also cause chronic focal ulcers that may bleed or perforate without warning symptoms .
	manualset3
117987	3	403824	13	NULL	NULL	0	NULL	acute diffuse injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonsteroidal anti-inflammatory drugs ( NSAIDs ) cause acute diffuse injury to the gastroduodenal mucosa , and also cause chronic focal ulcers that may bleed or perforate without warning symptoms .
	manualset3
117988	4	403824	13	NULL	NULL	0	NULL	 gastroduodenal mucosa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonsteroidal anti-inflammatory drugs ( NSAIDs ) cause acute diffuse injury to the gastroduodenal mucosa , and also cause chronic focal ulcers that may bleed or perforate without warning symptoms .
	manualset3
117989	5	403824	13	NULL	NULL	0	NULL	chronic focal ulcers	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonsteroidal anti-inflammatory drugs ( NSAIDs ) cause acute diffuse injury to the gastroduodenal mucosa , and also cause chronic focal ulcers that may bleed or perforate without warning symptoms .
	manualset3
117990	6	403824	13	NULL	NULL	0	NULL	warning symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonsteroidal anti-inflammatory drugs ( NSAIDs ) cause acute diffuse injury to the gastroduodenal mucosa , and also cause chronic focal ulcers that may bleed or perforate without warning symptoms .
	manualset3
117991	1	403825	13	NULL	NULL	0	NULL	Nonsteroidal anti-inflammatory drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonsteroidal anti-inflammatory drugs have been associated with hepatotoxicity in susceptible patients .
	manualset3
117992	2	403825	13	NULL	NULL	0	NULL	hepatotoxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonsteroidal anti-inflammatory drugs have been associated with hepatotoxicity in susceptible patients .
	manualset3
117993	3	403825	13	NULL	NULL	0	NULL	susceptible patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonsteroidal anti-inflammatory drugs have been associated with hepatotoxicity in susceptible patients .
	manualset3
117994	1	403826	13	NULL	NULL	0	NULL	Nonsurgical approaches	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonsurgical approaches to esophageal malignancy .
	manualset3
117995	2	403826	13	NULL	NULL	0	NULL	esophageal malignancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonsurgical approaches to esophageal malignancy .
	manualset3
117996	1	403827	13	NULL	NULL	0	NULL	spectrophotometric method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A continuous spectrophotometric method for monitoring phospholipase D-catalyzed hydrolysis of long acyl chain phosphatidylcholines has been formulated at pH 8.0 in a mixed detergent system using the coupling enzymes choline oxidase and peroxidase .
	manualset3
117997	2	403827	13	NULL	NULL	NULL	NULL	monitoring phospholipase D-catalyzed hydrolysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A continuous spectrophotometric method for monitoring phospholipase D-catalyzed hydrolysis of long acyl chain phosphatidylcholines has been formulated at pH 8.0 in a mixed detergent system using the coupling enzymes choline oxidase and peroxidase .
	manualset3
117999	4	403827	13	NULL	NULL	0	NULL	long acyl chain phosphatidylcholines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A continuous spectrophotometric method for monitoring phospholipase D-catalyzed hydrolysis of long acyl chain phosphatidylcholines has been formulated at pH 8.0 in a mixed detergent system using the coupling enzymes choline oxidase and peroxidase .
	manualset3
118000	5	403827	13	NULL	NULL	0	NULL	pH 8.0	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A continuous spectrophotometric method for monitoring phospholipase D-catalyzed hydrolysis of long acyl chain phosphatidylcholines has been formulated at pH 8.0 in a mixed detergent system using the coupling enzymes choline oxidase and peroxidase .
	manualset3
118001	6	403827	13	NULL	NULL	0	NULL	mixed detergent system	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A continuous spectrophotometric method for monitoring phospholipase D-catalyzed hydrolysis of long acyl chain phosphatidylcholines has been formulated at pH 8.0 in a mixed detergent system using the coupling enzymes choline oxidase and peroxidase .
	manualset3
118002	7	403827	13	NULL	NULL	0	NULL	coupling enzymes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A continuous spectrophotometric method for monitoring phospholipase D-catalyzed hydrolysis of long acyl chain phosphatidylcholines has been formulated at pH 8.0 in a mixed detergent system using the coupling enzymes choline oxidase and peroxidase .
	manualset3
118003	8	403827	13	NULL	NULL	0	NULL	choline oxidase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A continuous spectrophotometric method for monitoring phospholipase D-catalyzed hydrolysis of long acyl chain phosphatidylcholines has been formulated at pH 8.0 in a mixed detergent system using the coupling enzymes choline oxidase and peroxidase .
	manualset3
118004	9	403827	13	NULL	NULL	0	NULL	peroxidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A continuous spectrophotometric method for monitoring phospholipase D-catalyzed hydrolysis of long acyl chain phosphatidylcholines has been formulated at pH 8.0 in a mixed detergent system using the coupling enzymes choline oxidase and peroxidase .
	manualset3
118005	1	403828	13	NULL	NULL	0	NULL	Nonsynchronicity phenomenon	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonsynchronicity phenomenon observed during the lamellar-micellar phase transitions of 1-stearoyllysophosphatidylcholine dispersed in water .
	manualset3
118006	2	403828	13	NULL	NULL	0	NULL	lamellar-micellar phase transitions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonsynchronicity phenomenon observed during the lamellar-micellar phase transitions of 1-stearoyllysophosphatidylcholine dispersed in water .
	manualset3
118007	3	403828	13	NULL	NULL	0	NULL	1-stearoyllysophosphatidylcholine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonsynchronicity phenomenon observed during the lamellar-micellar phase transitions of 1-stearoyllysophosphatidylcholine dispersed in water .
	manualset3
118008	4	403828	13	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonsynchronicity phenomenon observed during the lamellar-micellar phase transitions of 1-stearoyllysophosphatidylcholine dispersed in water .
	manualset3
118009	1	403829	13	NULL	NULL	0	NULL	Nonverbal communication	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonverbal communication and modality of presentation had a significant effect on perception of leadership .
	manualset3
118010	2	403829	13	NULL	NULL	0	NULL	modality of presentation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonverbal communication and modality of presentation had a significant effect on perception of leadership .
	manualset3
118011	3	403829	13	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonverbal communication and modality of presentation had a significant effect on perception of leadership .
	manualset3
118012	4	403829	13	NULL	NULL	0	NULL	perception of leadership	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonverbal communication and modality of presentation had a significant effect on perception of leadership .
	manualset3
118013	1	403830	13	NULL	NULL	0	NULL	Noonan syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Noonan syndrome/leukemia-associated gain-of-function mutations in SHP-2 phosphatase ( PTPN11 ) enhance cell migration and angiogenesis .
	manualset3
118014	2	403830	13	NULL	NULL	0	NULL	leukemia-associated gain-of-function mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Noonan syndrome/leukemia-associated gain-of-function mutations in SHP-2 phosphatase ( PTPN11 ) enhance cell migration and angiogenesis .
	manualset3
118015	3	403830	13	NULL	NULL	0	NULL	SHP-2 phosphatase ( PTPN11 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Noonan syndrome/leukemia-associated gain-of-function mutations in SHP-2 phosphatase ( PTPN11 ) enhance cell migration and angiogenesis .
	manualset3
118016	4	403830	13	NULL	NULL	0	NULL	cell migration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Noonan syndrome/leukemia-associated gain-of-function mutations in SHP-2 phosphatase ( PTPN11 ) enhance cell migration and angiogenesis .
	manualset3
118017	5	403830	13	NULL	NULL	0	NULL	angiogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Noonan syndrome/leukemia-associated gain-of-function mutations in SHP-2 phosphatase ( PTPN11 ) enhance cell migration and angiogenesis .
	manualset3
118051	1	403831	13	NULL	NULL	0	NULL	Nor-BNI	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nor-BNI ( 4.9 nmol/mouse , i.c.v. ) did not block the effects of dynorphin A - ( 2-13 ) on the CO-induced impairment of learning and/or memory .
	manualset3
118052	2	403831	13	NULL	NULL	0	NULL	4.9 nmol/mouse , i.c.v.	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Nor-BNI ( 4.9 nmol/mouse , i.c.v. ) did not block the effects of dynorphin A - ( 2-13 ) on the CO-induced impairment of learning and/or memory .
	manualset3
118053	3	403831	13	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nor-BNI ( 4.9 nmol/mouse , i.c.v. ) did not block the effects of dynorphin A - ( 2-13 ) on the CO-induced impairment of learning and/or memory .
	manualset3
118054	4	403831	13	NULL	NULL	0	NULL	dynorphin A - ( 2-13 ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nor-BNI ( 4.9 nmol/mouse , i.c.v. ) did not block the effects of dynorphin A - ( 2-13 ) on the CO-induced impairment of learning and/or memory .
	manualset3
118055	5	403831	13	NULL	NULL	0	NULL	impairment of learning 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nor-BNI ( 4.9 nmol/mouse , i.c.v. ) did not block the effects of dynorphin A - ( 2-13 ) on the CO-induced impairment of learning and/or memory .
	manualset3
118056	6	403831	13	NULL	NULL	0	NULL	memory	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nor-BNI ( 4.9 nmol/mouse , i.c.v. ) did not block the effects of dynorphin A - ( 2-13 ) on the CO-induced impairment of learning and/or memory .
	manualset3
118057	1	403832	13	NULL	NULL	0	NULL	close relative	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Nor did having a close relative or friend with breast cancer affect the practice of BSE .
	manualset3
118058	2	403832	13	NULL	NULL	0	NULL	friend	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Nor did having a close relative or friend with breast cancer affect the practice of BSE .
	manualset3
118059	3	403832	13	NULL	NULL	0	NULL	breast cancer	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nor did having a close relative or friend with breast cancer affect the practice of BSE .
	manualset3
118060	4	403832	13	NULL	NULL	0	NULL	affect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nor did having a close relative or friend with breast cancer affect the practice of BSE .
	manualset3
118061	5	403832	13	NULL	NULL	0	NULL	practice of BSE	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nor did having a close relative or friend with breast cancer affect the practice of BSE .
	manualset3
118062	1	403833	13	NULL	NULL	0	NULL	soluble peptide 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Nor was the soluble peptide able to restore the loss of integrin-mediated cell adhesiveness to mini-laminin-332 after deletion of the gamma 2 chain C-terminus .
	manualset3
118063	2	403833	13	NULL	NULL	0	NULL	loss 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nor was the soluble peptide able to restore the loss of integrin-mediated cell adhesiveness to mini-laminin-332 after deletion of the gamma 2 chain C-terminus .
	manualset3
118064	3	403833	13	NULL	NULL	0	NULL	integrin-mediated cell adhesiveness 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nor was the soluble peptide able to restore the loss of integrin-mediated cell adhesiveness to mini-laminin-332 after deletion of the gamma 2 chain C-terminus .
	manualset3
118065	4	403833	13	NULL	NULL	0	NULL	mini-laminin-332	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nor was the soluble peptide able to restore the loss of integrin-mediated cell adhesiveness to mini-laminin-332 after deletion of the gamma 2 chain C-terminus .
	manualset3
118066	5	403833	13	NULL	NULL	0	NULL	deletion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nor was the soluble peptide able to restore the loss of integrin-mediated cell adhesiveness to mini-laminin-332 after deletion of the gamma 2 chain C-terminus .
	manualset3
118067	6	403833	13	NULL	NULL	0	NULL	gamma 2 chain C-terminus	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nor was the soluble peptide able to restore the loss of integrin-mediated cell adhesiveness to mini-laminin-332 after deletion of the gamma 2 chain C-terminus .
	manualset3
118068	1	403834	13	NULL	NULL	0	NULL	Noradrenaline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Noradrenaline and caffeine released 45Ca2 + from a cellular site in the aorta .
	manualset3
118069	2	403834	13	NULL	NULL	0	NULL	caffeine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Noradrenaline and caffeine released 45Ca2 + from a cellular site in the aorta .
	manualset3
118070	3	403834	13	NULL	NULL	0	NULL	45Ca2 + 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Noradrenaline and caffeine released 45Ca2 + from a cellular site in the aorta .
	manualset3
118071	4	403834	13	NULL	NULL	0	NULL	cellular site	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Noradrenaline and caffeine released 45Ca2 + from a cellular site in the aorta .
	manualset3
118072	5	403834	13	NULL	NULL	0	NULL	aorta	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Noradrenaline and caffeine released 45Ca2 + from a cellular site in the aorta .
	manualset3
118073	1	403835	13	NULL	NULL	0	NULL	Norepinephrine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Norepinephrine ( plus propranolol ) does not decrease the uptake or phosphorylation rate of ( methyl-14C ) choline .
	manualset3
118074	2	403835	13	NULL	NULL	0	NULL	propranolol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Norepinephrine ( plus propranolol ) does not decrease the uptake or phosphorylation rate of ( methyl-14C ) choline .
	manualset3
118075	3	403835	13	NULL	NULL	0	NULL	uptake 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Norepinephrine ( plus propranolol ) does not decrease the uptake or phosphorylation rate of ( methyl-14C ) choline .
	manualset3
118076	4	403835	13	NULL	NULL	0	NULL	phosphorylation rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Norepinephrine ( plus propranolol ) does not decrease the uptake or phosphorylation rate of ( methyl-14C ) choline .
	manualset3
118077	5	403835	13	NULL	NULL	0	NULL	( methyl-14C ) choline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Norepinephrine ( plus propranolol ) does not decrease the uptake or phosphorylation rate of ( methyl-14C ) choline .
	manualset3
118078	1	403836	13	NULL	NULL	0	NULL	Norepinephrine	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Norepinephrine , released from sympathetic neurons , and epinephrine , released from the adrenal medulla , participate in a number of physiological processes including those that facilitate adaptation to stressful conditions .
	manualset3
118079	2	403836	13	NULL	NULL	0	NULL	sympathetic neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Norepinephrine , released from sympathetic neurons , and epinephrine , released from the adrenal medulla , participate in a number of physiological processes including those that facilitate adaptation to stressful conditions .
	manualset3
118080	3	403836	13	NULL	NULL	0	NULL	epinephrine	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Norepinephrine , released from sympathetic neurons , and epinephrine , released from the adrenal medulla , participate in a number of physiological processes including those that facilitate adaptation to stressful conditions .
	manualset3
118081	4	403836	13	NULL	NULL	0	NULL	adrenal medulla	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Norepinephrine , released from sympathetic neurons , and epinephrine , released from the adrenal medulla , participate in a number of physiological processes including those that facilitate adaptation to stressful conditions .
	manualset3
118082	5	403836	13	NULL	NULL	0	NULL	number	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Norepinephrine , released from sympathetic neurons , and epinephrine , released from the adrenal medulla , participate in a number of physiological processes including those that facilitate adaptation to stressful conditions .
	manualset3
118083	6	403836	13	NULL	NULL	0	NULL	physiological processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Norepinephrine , released from sympathetic neurons , and epinephrine , released from the adrenal medulla , participate in a number of physiological processes including those that facilitate adaptation to stressful conditions .
	manualset3
118084	7	403836	13	NULL	NULL	0	NULL	adaptation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Norepinephrine , released from sympathetic neurons , and epinephrine , released from the adrenal medulla , participate in a number of physiological processes including those that facilitate adaptation to stressful conditions .
	manualset3
118085	8	403836	13	NULL	NULL	0	NULL	stressful conditions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Norepinephrine , released from sympathetic neurons , and epinephrine , released from the adrenal medulla , participate in a number of physiological processes including those that facilitate adaptation to stressful conditions .
	manualset3
118086	1	403837	13	NULL	NULL	0	NULL	Norepinephrine	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Norepinephrine induces VEGF expression and angiogenesis by a hypoxia-inducible factor-1 protein-dependent mechanism .
	manualset3
118087	2	403837	13	NULL	NULL	0	NULL	VEGF expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Norepinephrine induces VEGF expression and angiogenesis by a hypoxia-inducible factor-1 protein-dependent mechanism .
	manualset3
118088	3	403837	13	NULL	NULL	0	NULL	angiogenesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Norepinephrine induces VEGF expression and angiogenesis by a hypoxia-inducible factor-1 protein-dependent mechanism .
	manualset3
118089	4	403837	13	NULL	NULL	NULL	NULL	hypoxia-inducible factor-1 protein-dependent mechanism	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Norepinephrine induces VEGF expression and angiogenesis by a hypoxia-inducible factor-1 protein-dependent mechanism .
	manualset3
118090	1	403838	13	NULL	NULL	0	NULL	Normal rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal and adrenalectomized male rats were kept in 12 h light : 12 h dark ( 12L : 12 D ) or in constant light ( CL ) for 1 week .
	manualset3
118091	2	403838	13	NULL	NULL	0	NULL	adrenalectomized male rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal and adrenalectomized male rats were kept in 12 h light : 12 h dark ( 12L : 12 D ) or in constant light ( CL ) for 1 week .
	manualset3
118092	3	403838	13	NULL	NULL	NULL	NULL	12 h light : 12 h dark ( 12L : 12 D )	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Normal and adrenalectomized male rats were kept in 12 h light : 12 h dark ( 12L : 12 D ) or in constant light ( CL ) for 1 week .
	manualset3
118093	4	403838	13	NULL	NULL	NULL	NULL	constant light ( CL )	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Normal and adrenalectomized male rats were kept in 12 h light : 12 h dark ( 12L : 12 D ) or in constant light ( CL ) for 1 week .
	manualset3
118094	5	403838	13	NULL	NULL	0	NULL	1 week	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal and adrenalectomized male rats were kept in 12 h light : 12 h dark ( 12L : 12 D ) or in constant light ( CL ) for 1 week .
	manualset3
118095	1	403839	13	NULL	NULL	0	NULL	cytogenetics ( CN )	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal cytogenetics ( CN ) constitutes the single largest group , while trisomy 8 ( +8 ) as a sole abnormality is the most frequent trisomy .
	manualset3
118096	2	403839	13	NULL	NULL	0	NULL	group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal cytogenetics ( CN ) constitutes the single largest group , while trisomy 8 ( +8 ) as a sole abnormality is the most frequent trisomy .
	manualset3
118097	3	403839	13	NULL	NULL	0	NULL	trisomy 8 ( +8 )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal cytogenetics ( CN ) constitutes the single largest group , while trisomy 8 ( +8 ) as a sole abnormality is the most frequent trisomy .
	manualset3
118098	4	403839	13	NULL	NULL	0	NULL	sole abnormality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal cytogenetics ( CN ) constitutes the single largest group , while trisomy 8 ( +8 ) as a sole abnormality is the most frequent trisomy .
	manualset3
118099	5	403839	13	NULL	NULL	0	NULL	trisomy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal cytogenetics ( CN ) constitutes the single largest group , while trisomy 8 ( +8 ) as a sole abnormality is the most frequent trisomy .
	manualset3
118100	1	403840	13	NULL	NULL	0	NULL	Normal fasting gastrin levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal fasting gastrin levels do occur in patients with overt Zollinger-Ellison syndrome and should not deter further investigation if clinical suspicion of this syndrome is high .
	manualset3
118101	2	403840	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal fasting gastrin levels do occur in patients with overt Zollinger-Ellison syndrome and should not deter further investigation if clinical suspicion of this syndrome is high .
	manualset3
118102	3	403840	13	NULL	NULL	0	NULL	overt Zollinger-Ellison syndrome 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal fasting gastrin levels do occur in patients with overt Zollinger-Ellison syndrome and should not deter further investigation if clinical suspicion of this syndrome is high .
	manualset3
118103	4	403840	13	NULL	NULL	0	NULL	investigation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal fasting gastrin levels do occur in patients with overt Zollinger-Ellison syndrome and should not deter further investigation if clinical suspicion of this syndrome is high .
	manualset3
118104	5	403840	13	NULL	NULL	0	NULL	clinical suspicion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal fasting gastrin levels do occur in patients with overt Zollinger-Ellison syndrome and should not deter further investigation if clinical suspicion of this syndrome is high .
	manualset3
118105	6	403840	13	NULL	NULL	0	NULL	syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal fasting gastrin levels do occur in patients with overt Zollinger-Ellison syndrome and should not deter further investigation if clinical suspicion of this syndrome is high .
	manualset3
118196	1	403841	13	NULL	NULL	0	NULL	handling 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal handling of diets -- are all dogs created equal ?
	manualset3
118197	2	403841	13	NULL	NULL	0	NULL	diets	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal handling of diets -- are all dogs created equal ?
	manualset3
118198	3	403841	13	NULL	NULL	0	NULL	dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal handling of diets -- are all dogs created equal ?
	manualset3
118199	1	403842	13	NULL	NULL	0	NULL	Normal levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal levels of 2 , 3-diphosphoglycerate in red cells despite severe hypoxemia of chronic lung disease .
	manualset3
118200	2	403842	13	NULL	NULL	0	NULL	2 , 3-diphosphoglycerate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal levels of 2 , 3-diphosphoglycerate in red cells despite severe hypoxemia of chronic lung disease .
	manualset3
118201	3	403842	13	NULL	NULL	0	NULL	red cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal levels of 2 , 3-diphosphoglycerate in red cells despite severe hypoxemia of chronic lung disease .
	manualset3
118202	4	403842	13	NULL	NULL	0	NULL	hypoxemia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal levels of 2 , 3-diphosphoglycerate in red cells despite severe hypoxemia of chronic lung disease .
	manualset3
118203	5	403842	13	NULL	NULL	0	NULL	lung disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal levels of 2 , 3-diphosphoglycerate in red cells despite severe hypoxemia of chronic lung disease .
	manualset3
118204	1	403843	13	NULL	NULL	0	NULL	maturation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal maturation of the mammalian brain is characterized by periods of limitations in glucose transport capacity and increased use of alternative cerebral metabolic fuels such as lactate and ketone bodies , all of which are important during H/I and influence the development of energy failure .
	manualset3
118205	2	403843	13	NULL	NULL	0	NULL	mammalian brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal maturation of the mammalian brain is characterized by periods of limitations in glucose transport capacity and increased use of alternative cerebral metabolic fuels such as lactate and ketone bodies , all of which are important during H/I and influence the development of energy failure .
	manualset3
118206	3	403843	13	NULL	NULL	0	NULL	periods of limitations	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal maturation of the mammalian brain is characterized by periods of limitations in glucose transport capacity and increased use of alternative cerebral metabolic fuels such as lactate and ketone bodies , all of which are important during H/I and influence the development of energy failure .
	manualset3
118207	4	403843	13	NULL	NULL	0	NULL	glucose transport capacity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal maturation of the mammalian brain is characterized by periods of limitations in glucose transport capacity and increased use of alternative cerebral metabolic fuels such as lactate and ketone bodies , all of which are important during H/I and influence the development of energy failure .
	manualset3
118208	5	403843	13	NULL	NULL	0	NULL	alternative cerebral metabolic fuels 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal maturation of the mammalian brain is characterized by periods of limitations in glucose transport capacity and increased use of alternative cerebral metabolic fuels such as lactate and ketone bodies , all of which are important during H/I and influence the development of energy failure .
	manualset3
118209	6	403843	13	NULL	NULL	0	NULL	lactate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal maturation of the mammalian brain is characterized by periods of limitations in glucose transport capacity and increased use of alternative cerebral metabolic fuels such as lactate and ketone bodies , all of which are important during H/I and influence the development of energy failure .
	manualset3
118210	7	403843	13	NULL	NULL	0	NULL	ketone bodies	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal maturation of the mammalian brain is characterized by periods of limitations in glucose transport capacity and increased use of alternative cerebral metabolic fuels such as lactate and ketone bodies , all of which are important during H/I and influence the development of energy failure .
	manualset3
118211	8	403843	13	NULL	NULL	0	NULL	H/I 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal maturation of the mammalian brain is characterized by periods of limitations in glucose transport capacity and increased use of alternative cerebral metabolic fuels such as lactate and ketone bodies , all of which are important during H/I and influence the development of energy failure .
	manualset3
118212	9	403843	13	NULL	NULL	0	NULL	development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal maturation of the mammalian brain is characterized by periods of limitations in glucose transport capacity and increased use of alternative cerebral metabolic fuels such as lactate and ketone bodies , all of which are important during H/I and influence the development of energy failure .
	manualset3
118213	10	403843	13	NULL	NULL	0	NULL	energy failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal maturation of the mammalian brain is characterized by periods of limitations in glucose transport capacity and increased use of alternative cerebral metabolic fuels such as lactate and ketone bodies , all of which are important during H/I and influence the development of energy failure .
	manualset3
118214	1	403844	13	NULL	NULL	NULL	NULL	motion	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Normal motion is 3-dimensional , and during arm elevation consists of upward rotation , posterior tilting , and external rotation as well as clavicular elevation and retraction .
	manualset3
118215	2	403844	13	NULL	NULL	NULL	NULL	arm elevation 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Normal motion is 3-dimensional , and during arm elevation consists of upward rotation , posterior tilting , and external rotation as well as clavicular elevation and retraction .
	manualset3
118216	3	403844	13	NULL	NULL	NULL	NULL	upward rotation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Normal motion is 3-dimensional , and during arm elevation consists of upward rotation , posterior tilting , and external rotation as well as clavicular elevation and retraction .
	manualset3
118217	4	403844	13	NULL	NULL	NULL	NULL	posterior tilting 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Normal motion is 3-dimensional , and during arm elevation consists of upward rotation , posterior tilting , and external rotation as well as clavicular elevation and retraction .
	manualset3
118218	5	403844	13	NULL	NULL	NULL	NULL	external rotation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Normal motion is 3-dimensional , and during arm elevation consists of upward rotation , posterior tilting , and external rotation as well as clavicular elevation and retraction .
	manualset3
118219	6	403844	13	NULL	NULL	NULL	NULL	clavicular elevation 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Normal motion is 3-dimensional , and during arm elevation consists of upward rotation , posterior tilting , and external rotation as well as clavicular elevation and retraction .
	manualset3
118280	7	403844	13	NULL	NULL	NULL	NULL	retraction	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Normal motion is 3-dimensional , and during arm elevation consists of upward rotation , posterior tilting , and external rotation as well as clavicular elevation and retraction .
	manualset3
118299	1	403845	13	NULL	NULL	0	NULL	cerebral blood flow	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal newborn cerebral blood flow is low ; fetal asphyxia at birth causes delayed cerebral hyperperfusion in the neonate .
	manualset3
118300	2	403845	13	NULL	NULL	0	NULL	fetal asphyxia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal newborn cerebral blood flow is low ; fetal asphyxia at birth causes delayed cerebral hyperperfusion in the neonate .
	manualset3
118301	3	403845	13	NULL	NULL	0	NULL	birth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal newborn cerebral blood flow is low ; fetal asphyxia at birth causes delayed cerebral hyperperfusion in the neonate .
	manualset3
118303	4	403845	13	NULL	NULL	0	NULL	causes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal newborn cerebral blood flow is low ; fetal asphyxia at birth causes delayed cerebral hyperperfusion in the neonate .
	manualset3
118316	5	403845	13	NULL	NULL	0	NULL	 cerebral hyperperfusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal newborn cerebral blood flow is low ; fetal asphyxia at birth causes delayed cerebral hyperperfusion in the neonate .
	manualset3
118317	6	403845	13	NULL	NULL	0	NULL	neonate	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal newborn cerebral blood flow is low ; fetal asphyxia at birth causes delayed cerebral hyperperfusion in the neonate .
	manualset3
118318	1	403846	13	NULL	NULL	0	NULL	Normal platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal platelets are known to have NOS activity , but little is known about NOS expression and NO production by platelets in patients with IPAH .
	manualset3
118319	2	403846	13	NULL	NULL	0	NULL	NOS activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal platelets are known to have NOS activity , but little is known about NOS expression and NO production by platelets in patients with IPAH .
	manualset3
118320	3	403846	13	NULL	NULL	0	NULL	NOS expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal platelets are known to have NOS activity , but little is known about NOS expression and NO production by platelets in patients with IPAH .
	manualset3
118321	4	403846	13	NULL	NULL	0	NULL	NO production 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal platelets are known to have NOS activity , but little is known about NOS expression and NO production by platelets in patients with IPAH .
	manualset3
118322	5	403846	13	NULL	NULL	0	NULL	platelets 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal platelets are known to have NOS activity , but little is known about NOS expression and NO production by platelets in patients with IPAH .
	manualset3
118323	6	403846	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal platelets are known to have NOS activity , but little is known about NOS expression and NO production by platelets in patients with IPAH .
	manualset3
118324	7	403846	13	NULL	NULL	0	NULL	IPAH 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal platelets are known to have NOS activity , but little is known about NOS expression and NO production by platelets in patients with IPAH .
	manualset3
118337	1	403847	13	NULL	NULL	0	NULL	size	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal size left ventricle on antenatal scan in lethal hypoplastic left heart syndrome .
	manualset3
118339	2	403847	13	NULL	NULL	0	NULL	left ventricle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal size left ventricle on antenatal scan in lethal hypoplastic left heart syndrome .
	manualset3
118340	3	403847	13	NULL	NULL	0	NULL	antenatal scan 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal size left ventricle on antenatal scan in lethal hypoplastic left heart syndrome .
	manualset3
118343	4	403847	13	NULL	NULL	0	NULL	lethal hypoplastic left heart syndrome 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal size left ventricle on antenatal scan in lethal hypoplastic left heart syndrome .
	manualset3
118373	1	403848	13	NULL	NULL	0	NULL	contribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A contribution to natural childbirth ) .
	manualset3
118374	2	403848	13	NULL	NULL	0	NULL	natural childbirth 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A contribution to natural childbirth ) .
	manualset3
118384	1	403849	13	NULL	NULL	0	NULL	strains 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal strains release fragments comparable in amount to the DNA taken up ; but , in a mutant selected for inability to degrade DNA in agar , the amount of fragments formed external to the cells is only 40 % of DNA uptake .
	manualset3
118386	3	403849	13	NULL	NULL	0	NULL	fragments	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal strains release fragments comparable in amount to the DNA taken up ; but , in a mutant selected for inability to degrade DNA in agar , the amount of fragments formed external to the cells is only 40 % of DNA uptake .
	manualset3
118387	4	403849	13	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal strains release fragments comparable in amount to the DNA taken up ; but , in a mutant selected for inability to degrade DNA in agar , the amount of fragments formed external to the cells is only 40 % of DNA uptake .
	manualset3
118389	5	403849	13	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal strains release fragments comparable in amount to the DNA taken up ; but , in a mutant selected for inability to degrade DNA in agar , the amount of fragments formed external to the cells is only 40 % of DNA uptake .
	manualset3
118390	6	403849	13	NULL	NULL	0	NULL	mutant 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal strains release fragments comparable in amount to the DNA taken up ; but , in a mutant selected for inability to degrade DNA in agar , the amount of fragments formed external to the cells is only 40 % of DNA uptake .
	manualset3
118391	7	403849	13	NULL	NULL	0	NULL	inability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal strains release fragments comparable in amount to the DNA taken up ; but , in a mutant selected for inability to degrade DNA in agar , the amount of fragments formed external to the cells is only 40 % of DNA uptake .
	manualset3
118392	8	403849	13	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal strains release fragments comparable in amount to the DNA taken up ; but , in a mutant selected for inability to degrade DNA in agar , the amount of fragments formed external to the cells is only 40 % of DNA uptake .
	manualset3
118394	9	403849	13	NULL	NULL	0	NULL	agar 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal strains release fragments comparable in amount to the DNA taken up ; but , in a mutant selected for inability to degrade DNA in agar , the amount of fragments formed external to the cells is only 40 % of DNA uptake .
	manualset3
118395	10	403849	13	NULL	NULL	0	NULL	amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal strains release fragments comparable in amount to the DNA taken up ; but , in a mutant selected for inability to degrade DNA in agar , the amount of fragments formed external to the cells is only 40 % of DNA uptake .
	manualset3
118397	11	403849	13	NULL	NULL	0	NULL	fragments	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal strains release fragments comparable in amount to the DNA taken up ; but , in a mutant selected for inability to degrade DNA in agar , the amount of fragments formed external to the cells is only 40 % of DNA uptake .
	manualset3
118399	12	403849	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal strains release fragments comparable in amount to the DNA taken up ; but , in a mutant selected for inability to degrade DNA in agar , the amount of fragments formed external to the cells is only 40 % of DNA uptake .
	manualset3
118400	13	403849	13	NULL	NULL	0	NULL	40 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal strains release fragments comparable in amount to the DNA taken up ; but , in a mutant selected for inability to degrade DNA in agar , the amount of fragments formed external to the cells is only 40 % of DNA uptake .
	manualset3
118402	14	403849	13	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal strains release fragments comparable in amount to the DNA taken up ; but , in a mutant selected for inability to degrade DNA in agar , the amount of fragments formed external to the cells is only 40 % of DNA uptake .
	manualset3
118403	15	403849	13	NULL	NULL	0	NULL	uptake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Normal strains release fragments comparable in amount to the DNA taken up ; but , in a mutant selected for inability to degrade DNA in agar , the amount of fragments formed external to the cells is only 40 % of DNA uptake .
	manualset3
118406	1	403850	13	NULL	NULL	0	NULL	Normalization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Normalization of hemoglobin in incident hemodialysis patients does not have a beneficial effect on cardiac structure , compared with partial correction .
	manualset3
118410	2	403850	13	NULL	NULL	0	NULL	hemoglobin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Normalization of hemoglobin in incident hemodialysis patients does not have a beneficial effect on cardiac structure , compared with partial correction .
	manualset3
118414	3	403850	13	NULL	NULL	0	NULL	incident hemodialysis patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Normalization of hemoglobin in incident hemodialysis patients does not have a beneficial effect on cardiac structure , compared with partial correction .
	manualset3
118415	4	403850	13	NULL	NULL	0	NULL	beneficial effect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Normalization of hemoglobin in incident hemodialysis patients does not have a beneficial effect on cardiac structure , compared with partial correction .
	manualset3
118418	5	403850	13	NULL	NULL	0	NULL	cardiac structure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Normalization of hemoglobin in incident hemodialysis patients does not have a beneficial effect on cardiac structure , compared with partial correction .
	manualset3
118420	6	403850	13	NULL	NULL	0	NULL	partial correction 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Normalization of hemoglobin in incident hemodialysis patients does not have a beneficial effect on cardiac structure , compared with partial correction .
	manualset3
118425	1	403851	13	NULL	NULL	0	NULL	Northern analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Northern analysis revealed that neugrin was strongly expressed in the heart , brain , and skeletal muscle , and m-neugrin in the liver , kidney , and brain .
	manualset3
118428	2	403851	13	NULL	NULL	0	NULL	neugrin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Northern analysis revealed that neugrin was strongly expressed in the heart , brain , and skeletal muscle , and m-neugrin in the liver , kidney , and brain .
	manualset3
118429	3	403851	13	NULL	NULL	0	NULL	heart	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Northern analysis revealed that neugrin was strongly expressed in the heart , brain , and skeletal muscle , and m-neugrin in the liver , kidney , and brain .
	manualset3
118430	4	403851	13	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Northern analysis revealed that neugrin was strongly expressed in the heart , brain , and skeletal muscle , and m-neugrin in the liver , kidney , and brain .
	manualset3
118432	5	403851	13	NULL	NULL	0	NULL	skeletal muscle 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Northern analysis revealed that neugrin was strongly expressed in the heart , brain , and skeletal muscle , and m-neugrin in the liver , kidney , and brain .
	manualset3
118433	6	403851	13	NULL	NULL	0	NULL	m-neugrin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Northern analysis revealed that neugrin was strongly expressed in the heart , brain , and skeletal muscle , and m-neugrin in the liver , kidney , and brain .
	manualset3
118434	7	403851	13	NULL	NULL	0	NULL	liver 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Northern analysis revealed that neugrin was strongly expressed in the heart , brain , and skeletal muscle , and m-neugrin in the liver , kidney , and brain .
	manualset3
118435	8	403851	13	NULL	NULL	0	NULL	kidney	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Northern analysis revealed that neugrin was strongly expressed in the heart , brain , and skeletal muscle , and m-neugrin in the liver , kidney , and brain .
	manualset3
118436	9	403851	13	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Northern analysis revealed that neugrin was strongly expressed in the heart , brain , and skeletal muscle , and m-neugrin in the liver , kidney , and brain .
	manualset3
118438	1	403852	13	NULL	NULL	0	NULL	Northern analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Northern and Western blot analysis indicated that Nogo-A is predominantly expressed in the nervous system with lower levels also present in testis and heart .
	manualset3
118439	2	403852	13	NULL	NULL	0	NULL	Western blot analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Northern and Western blot analysis indicated that Nogo-A is predominantly expressed in the nervous system with lower levels also present in testis and heart .
	manualset3
118441	3	403852	13	NULL	NULL	0	NULL	Nogo-A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Northern and Western blot analysis indicated that Nogo-A is predominantly expressed in the nervous system with lower levels also present in testis and heart .
	manualset3
118443	4	403852	13	NULL	NULL	0	NULL	nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Northern and Western blot analysis indicated that Nogo-A is predominantly expressed in the nervous system with lower levels also present in testis and heart .
	manualset3
118446	5	403852	13	NULL	NULL	0	NULL	levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Northern and Western blot analysis indicated that Nogo-A is predominantly expressed in the nervous system with lower levels also present in testis and heart .
	manualset3
118448	6	403852	13	NULL	NULL	0	NULL	testis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Northern and Western blot analysis indicated that Nogo-A is predominantly expressed in the nervous system with lower levels also present in testis and heart .
	manualset3
118449	7	403852	13	NULL	NULL	0	NULL	heart	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Northern and Western blot analysis indicated that Nogo-A is predominantly expressed in the nervous system with lower levels also present in testis and heart .
	manualset3
118455	1	403853	13	NULL	NULL	0	NULL	Northern analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Northern analyses with riboprobes derived from the delta and kappa opioid receptor clones indicate these sequences are expressed at low levels in human peripheral blood lymphocytes and in several human lymphoid cell lines .
	manualset3
118461	2	403853	13	NULL	NULL	0	NULL	riboprobes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Northern analyses with riboprobes derived from the delta and kappa opioid receptor clones indicate these sequences are expressed at low levels in human peripheral blood lymphocytes and in several human lymphoid cell lines .
	manualset3
118462	3	403853	13	NULL	NULL	NULL	NULL	delta opioid receptor clone	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Northern analyses with riboprobes derived from the delta and kappa opioid receptor clones indicate these sequences are expressed at low levels in human peripheral blood lymphocytes and in several human lymphoid cell lines .
	manualset3
118463	4	403853	13	NULL	NULL	0	NULL	kappa opioid receptor clone	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Northern analyses with riboprobes derived from the delta and kappa opioid receptor clones indicate these sequences are expressed at low levels in human peripheral blood lymphocytes and in several human lymphoid cell lines .
	manualset3
118466	5	403853	13	NULL	NULL	0	NULL	sequences 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Northern analyses with riboprobes derived from the delta and kappa opioid receptor clones indicate these sequences are expressed at low levels in human peripheral blood lymphocytes and in several human lymphoid cell lines .
	manualset3
118469	6	403853	13	NULL	NULL	0	NULL	levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Northern analyses with riboprobes derived from the delta and kappa opioid receptor clones indicate these sequences are expressed at low levels in human peripheral blood lymphocytes and in several human lymphoid cell lines .
	manualset3
118470	7	403853	13	NULL	NULL	0	NULL	human peripheral blood lymphocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Northern analyses with riboprobes derived from the delta and kappa opioid receptor clones indicate these sequences are expressed at low levels in human peripheral blood lymphocytes and in several human lymphoid cell lines .
	manualset3
118472	8	403853	13	NULL	NULL	0	NULL	several human lymphoid cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Northern analyses with riboprobes derived from the delta and kappa opioid receptor clones indicate these sequences are expressed at low levels in human peripheral blood lymphocytes and in several human lymphoid cell lines .
	manualset3
118473	1	403854	13	NULL	NULL	0	NULL	Northwest Ohio hospitals	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Northwest Ohio hospitals plan partnership .
	manualset3
118475	2	403854	13	NULL	NULL	0	NULL	partnership	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Northwest Ohio hospitals plan partnership .
	manualset3
118477	1	403855	13	NULL	NULL	0	NULL	control group of patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A control group of patients who underwent varicose vein surgery to the groin under general anesthetic without any muscle dissection demonstrated no alteration in response times .
	manualset3
118478	2	403855	13	NULL	NULL	0	NULL	varicose vein surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A control group of patients who underwent varicose vein surgery to the groin under general anesthetic without any muscle dissection demonstrated no alteration in response times .
	manualset3
118479	3	403855	13	NULL	NULL	0	NULL	groin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A control group of patients who underwent varicose vein surgery to the groin under general anesthetic without any muscle dissection demonstrated no alteration in response times .
	manualset3
118485	4	403855	13	NULL	NULL	0	NULL	general anesthetic 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A control group of patients who underwent varicose vein surgery to the groin under general anesthetic without any muscle dissection demonstrated no alteration in response times .
	manualset3
118487	5	403855	13	NULL	NULL	0	NULL	muscle dissection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A control group of patients who underwent varicose vein surgery to the groin under general anesthetic without any muscle dissection demonstrated no alteration in response times .
	manualset3
118489	6	403855	13	NULL	NULL	0	NULL	alteration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A control group of patients who underwent varicose vein surgery to the groin under general anesthetic without any muscle dissection demonstrated no alteration in response times .
	manualset3
118490	7	403855	13	NULL	NULL	0	NULL	response times	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A control group of patients who underwent varicose vein surgery to the groin under general anesthetic without any muscle dissection demonstrated no alteration in response times .
	manualset3
118491	1	403856	13	NULL	NULL	0	NULL	11-9-1-4 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Not only did 11-9-1-4 express galectin-3 in the usual punctate pattern on its cell surface , it demonstrated a higher surface expression of alpha 6 beta 1 integrin compared to BT-549 .
	manualset3
118495	2	403856	13	NULL	NULL	0	NULL	galectin-3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Not only did 11-9-1-4 express galectin-3 in the usual punctate pattern on its cell surface , it demonstrated a higher surface expression of alpha 6 beta 1 integrin compared to BT-549 .
	manualset3
118496	3	403856	13	NULL	NULL	0	NULL	punctate pattern 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Not only did 11-9-1-4 express galectin-3 in the usual punctate pattern on its cell surface , it demonstrated a higher surface expression of alpha 6 beta 1 integrin compared to BT-549 .
	manualset3
118497	4	403856	13	NULL	NULL	0	NULL	cell surface	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Not only did 11-9-1-4 express galectin-3 in the usual punctate pattern on its cell surface , it demonstrated a higher surface expression of alpha 6 beta 1 integrin compared to BT-549 .
	manualset3
118498	5	403856	13	NULL	NULL	0	NULL	surface expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Not only did 11-9-1-4 express galectin-3 in the usual punctate pattern on its cell surface , it demonstrated a higher surface expression of alpha 6 beta 1 integrin compared to BT-549 .
	manualset3
118499	6	403856	13	NULL	NULL	0	NULL	alpha 6 beta 1 integrin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Not only did 11-9-1-4 express galectin-3 in the usual punctate pattern on its cell surface , it demonstrated a higher surface expression of alpha 6 beta 1 integrin compared to BT-549 .
	manualset3
118500	7	403856	13	NULL	NULL	0	NULL	BT-549	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Not only did 11-9-1-4 express galectin-3 in the usual punctate pattern on its cell surface , it demonstrated a higher surface expression of alpha 6 beta 1 integrin compared to BT-549 .
	manualset3
118505	1	403857	13	NULL	NULL	0	NULL	investigators	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Not surprising , investigators of Alzheimer 's disease have also evaluated adult neurogenesis due to its responsiveness to hippocampal damage .
	manualset3
118506	2	403857	13	NULL	NULL	0	NULL	Alzheimer 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Not surprising , investigators of Alzheimer 's disease have also evaluated adult neurogenesis due to its responsiveness to hippocampal damage .
	manualset3
118507	3	403857	13	NULL	NULL	0	NULL	adult neurogenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Not surprising , investigators of Alzheimer 's disease have also evaluated adult neurogenesis due to its responsiveness to hippocampal damage .
	manualset3
118509	4	403857	13	NULL	NULL	0	NULL	responsiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Not surprising , investigators of Alzheimer 's disease have also evaluated adult neurogenesis due to its responsiveness to hippocampal damage .
	manualset3
118511	5	403857	13	NULL	NULL	0	NULL	hippocampal damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Not surprising , investigators of Alzheimer 's disease have also evaluated adult neurogenesis due to its responsiveness to hippocampal damage .
	manualset3
118521	1	403858	13	NULL	NULL	0	NULL	ARD1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , ARD1 was critical for transcriptionally regulating a number of AR target genes that are involved in prostate tumorigenesis .
	manualset3
118523	2	403858	13	NULL	NULL	0	NULL	number	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , ARD1 was critical for transcriptionally regulating a number of AR target genes that are involved in prostate tumorigenesis .
	manualset3
118525	3	403858	13	NULL	NULL	0	NULL	AR target genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , ARD1 was critical for transcriptionally regulating a number of AR target genes that are involved in prostate tumorigenesis .
	manualset3
118527	4	403858	13	NULL	NULL	0	NULL	prostate tumorigenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , ARD1 was critical for transcriptionally regulating a number of AR target genes that are involved in prostate tumorigenesis .
	manualset3
118532	1	403859	13	NULL	NULL	0	NULL	CRF rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , CRF rats eating 30 % protein had the lowest protein efficiency ; their calorie intake was also the lowest because of anorexia .
	manualset3
118534	2	403859	13	NULL	NULL	0	NULL	30 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , CRF rats eating 30 % protein had the lowest protein efficiency ; their calorie intake was also the lowest because of anorexia .
	manualset3
118536	3	403859	13	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , CRF rats eating 30 % protein had the lowest protein efficiency ; their calorie intake was also the lowest because of anorexia .
	manualset3
118538	4	403859	13	NULL	NULL	0	NULL	protein efficiency	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , CRF rats eating 30 % protein had the lowest protein efficiency ; their calorie intake was also the lowest because of anorexia .
	manualset3
118539	5	403859	13	NULL	NULL	0	NULL	calorie	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , CRF rats eating 30 % protein had the lowest protein efficiency ; their calorie intake was also the lowest because of anorexia .
	manualset3
118540	6	403859	13	NULL	NULL	0	NULL	intake 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , CRF rats eating 30 % protein had the lowest protein efficiency ; their calorie intake was also the lowest because of anorexia .
	manualset3
118541	7	403859	13	NULL	NULL	0	NULL	anorexia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , CRF rats eating 30 % protein had the lowest protein efficiency ; their calorie intake was also the lowest because of anorexia .
	manualset3
118542	1	403860	13	NULL	NULL	0	NULL	HCV-JFH1 infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , HCV-JFH1 infection also redistributed the stress granule components GTPase-activating protein ( SH3 domain ) - binding protein 1 ( G3BP1 ) , ataxin-2 ( ATX2 ) , and poly ( A ) - binding protein 1 ( PABP1 ) to the HCV production factory .
	manualset3
118543	2	403860	13	NULL	NULL	0	NULL	 stress granule components	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , HCV-JFH1 infection also redistributed the stress granule components GTPase-activating protein ( SH3 domain ) - binding protein 1 ( G3BP1 ) , ataxin-2 ( ATX2 ) , and poly ( A ) - binding protein 1 ( PABP1 ) to the HCV production factory .
	manualset3
118544	3	403860	13	NULL	NULL	0	NULL	GTPase-activating protein ( SH3 domain ) - binding protein 1 ( G3BP1 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , HCV-JFH1 infection also redistributed the stress granule components GTPase-activating protein ( SH3 domain ) - binding protein 1 ( G3BP1 ) , ataxin-2 ( ATX2 ) , and poly ( A ) - binding protein 1 ( PABP1 ) to the HCV production factory .
	manualset3
118546	4	403860	13	NULL	NULL	0	NULL	ataxin-2 ( ATX2 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , HCV-JFH1 infection also redistributed the stress granule components GTPase-activating protein ( SH3 domain ) - binding protein 1 ( G3BP1 ) , ataxin-2 ( ATX2 ) , and poly ( A ) - binding protein 1 ( PABP1 ) to the HCV production factory .
	manualset3
118548	5	403860	13	NULL	NULL	0	NULL	poly ( A ) - binding protein 1 ( PABP1 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , HCV-JFH1 infection also redistributed the stress granule components GTPase-activating protein ( SH3 domain ) - binding protein 1 ( G3BP1 ) , ataxin-2 ( ATX2 ) , and poly ( A ) - binding protein 1 ( PABP1 ) to the HCV production factory .
	manualset3
118549	6	403860	13	NULL	NULL	0	NULL	HCV production factory	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , HCV-JFH1 infection also redistributed the stress granule components GTPase-activating protein ( SH3 domain ) - binding protein 1 ( G3BP1 ) , ataxin-2 ( ATX2 ) , and poly ( A ) - binding protein 1 ( PABP1 ) to the HCV production factory .
	manualset3
118559	1	403861	13	NULL	NULL	0	NULL	HDAC inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , HDAC inhibitors led to noticeable HDAC4 degradation , which was effectively prevented by MG132 .
	manualset3
118560	2	403861	13	NULL	NULL	0	NULL	HDAC4 degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , HDAC inhibitors led to noticeable HDAC4 degradation , which was effectively prevented by MG132 .
	manualset3
118561	3	403861	13	NULL	NULL	0	NULL	MG132	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , HDAC inhibitors led to noticeable HDAC4 degradation , which was effectively prevented by MG132 .
	manualset3
118562	1	403862	13	NULL	NULL	0	NULL	three 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , all three polymorphisms analyzed were associated ( P0 .05 ) with at least one of a number of performance traits related to animal body size : angularity , body depth , chest width , rump width , and animal stature .
	manualset3
118563	2	403862	13	NULL	NULL	0	NULL	polymorphisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , all three polymorphisms analyzed were associated ( P0 .05 ) with at least one of a number of performance traits related to animal body size : angularity , body depth , chest width , rump width , and animal stature .
	manualset3
118564	3	403862	13	NULL	NULL	0	NULL	P0 .05 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , all three polymorphisms analyzed were associated ( P0 .05 ) with at least one of a number of performance traits related to animal body size : angularity , body depth , chest width , rump width , and animal stature .
	manualset3
118565	4	403862	13	NULL	NULL	0	NULL	number	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , all three polymorphisms analyzed were associated ( P0 .05 ) with at least one of a number of performance traits related to animal body size : angularity , body depth , chest width , rump width , and animal stature .
	manualset3
118566	5	403862	13	NULL	NULL	0	NULL	performance traits	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , all three polymorphisms analyzed were associated ( P0 .05 ) with at least one of a number of performance traits related to animal body size : angularity , body depth , chest width , rump width , and animal stature .
	manualset3
118567	6	403862	13	NULL	NULL	0	NULL	animal body size	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , all three polymorphisms analyzed were associated ( P0 .05 ) with at least one of a number of performance traits related to animal body size : angularity , body depth , chest width , rump width , and animal stature .
	manualset3
118568	7	403862	13	NULL	NULL	0	NULL	angularity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , all three polymorphisms analyzed were associated ( P0 .05 ) with at least one of a number of performance traits related to animal body size : angularity , body depth , chest width , rump width , and animal stature .
	manualset3
118569	8	403862	13	NULL	NULL	0	NULL	body depth	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , all three polymorphisms analyzed were associated ( P0 .05 ) with at least one of a number of performance traits related to animal body size : angularity , body depth , chest width , rump width , and animal stature .
	manualset3
118570	9	403862	13	NULL	NULL	0	NULL	chest width 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , all three polymorphisms analyzed were associated ( P0 .05 ) with at least one of a number of performance traits related to animal body size : angularity , body depth , chest width , rump width , and animal stature .
	manualset3
118571	10	403862	13	NULL	NULL	0	NULL	rump width	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , all three polymorphisms analyzed were associated ( P0 .05 ) with at least one of a number of performance traits related to animal body size : angularity , body depth , chest width , rump width , and animal stature .
	manualset3
118572	11	403862	13	NULL	NULL	NULL	NULL	animal stature 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Notably , all three polymorphisms analyzed were associated ( P0 .05 ) with at least one of a number of performance traits related to animal body size : angularity , body depth , chest width , rump width , and animal stature .
	manualset3
118573	1	403863	13	NULL	NULL	0	NULL	changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , changes in serotonin turnover developed on the contralateral side .
	manualset3
118574	2	403863	13	NULL	NULL	0	NULL	serotonin turnover	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , changes in serotonin turnover developed on the contralateral side .
	manualset3
118575	3	403863	13	NULL	NULL	0	NULL	contralateral side	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , changes in serotonin turnover developed on the contralateral side .
	manualset3
118576	1	403864	13	NULL	NULL	0	NULL	heparanase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , heparanase stimulates macrophage activation , while macrophages induce production and activation of latent heparanase contributed by the colon epithelium , together generating a vicious cycle that powers colitis and the associated tumorigenesis .
	manualset3
118577	2	403864	13	NULL	NULL	0	NULL	 macrophage activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , heparanase stimulates macrophage activation , while macrophages induce production and activation of latent heparanase contributed by the colon epithelium , together generating a vicious cycle that powers colitis and the associated tumorigenesis .
	manualset3
118578	3	403864	13	NULL	NULL	0	NULL	macrophages 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , heparanase stimulates macrophage activation , while macrophages induce production and activation of latent heparanase contributed by the colon epithelium , together generating a vicious cycle that powers colitis and the associated tumorigenesis .
	manualset3
118579	4	403864	13	NULL	NULL	NULL	NULL	production	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Notably , heparanase stimulates macrophage activation , while macrophages induce production and activation of latent heparanase contributed by the colon epithelium , together generating a vicious cycle that powers colitis and the associated tumorigenesis .
	manualset3
118580	5	403864	13	NULL	NULL	0	NULL	activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , heparanase stimulates macrophage activation , while macrophages induce production and activation of latent heparanase contributed by the colon epithelium , together generating a vicious cycle that powers colitis and the associated tumorigenesis .
	manualset3
118581	6	403864	13	NULL	NULL	0	NULL	latent heparanase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , heparanase stimulates macrophage activation , while macrophages induce production and activation of latent heparanase contributed by the colon epithelium , together generating a vicious cycle that powers colitis and the associated tumorigenesis .
	manualset3
118582	7	403864	13	NULL	NULL	0	NULL	colon epithelium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , heparanase stimulates macrophage activation , while macrophages induce production and activation of latent heparanase contributed by the colon epithelium , together generating a vicious cycle that powers colitis and the associated tumorigenesis .
	manualset3
118583	8	403864	13	NULL	NULL	0	NULL	vicious cycle	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , heparanase stimulates macrophage activation , while macrophages induce production and activation of latent heparanase contributed by the colon epithelium , together generating a vicious cycle that powers colitis and the associated tumorigenesis .
	manualset3
118584	9	403864	13	NULL	NULL	0	NULL	colitis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , heparanase stimulates macrophage activation , while macrophages induce production and activation of latent heparanase contributed by the colon epithelium , together generating a vicious cycle that powers colitis and the associated tumorigenesis .
	manualset3
118585	10	403864	13	NULL	NULL	0	NULL	tumorigenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , heparanase stimulates macrophage activation , while macrophages induce production and activation of latent heparanase contributed by the colon epithelium , together generating a vicious cycle that powers colitis and the associated tumorigenesis .
	manualset3
118586	1	403865	13	NULL	NULL	0	NULL	water soluble multihoppers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , no lag is predicted for less water soluble multihoppers ( K ( AW ) ) 1 ) , which are more likely to distribute into soils and foliage , because the terrestrial environment is `` stickier '' than the oceans , greatly reducing the number of hops these chemical will experience .
	manualset3
118587	2	403865	13	NULL	NULL	0	NULL	K ( AW ) ) 1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , no lag is predicted for less water soluble multihoppers ( K ( AW ) ) 1 ) , which are more likely to distribute into soils and foliage , because the terrestrial environment is `` stickier '' than the oceans , greatly reducing the number of hops these chemical will experience .
	manualset3
118588	3	403865	13	NULL	NULL	0	NULL	soils	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , no lag is predicted for less water soluble multihoppers ( K ( AW ) ) 1 ) , which are more likely to distribute into soils and foliage , because the terrestrial environment is `` stickier '' than the oceans , greatly reducing the number of hops these chemical will experience .
	manualset3
118589	4	403865	13	NULL	NULL	0	NULL	foliage	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , no lag is predicted for less water soluble multihoppers ( K ( AW ) ) 1 ) , which are more likely to distribute into soils and foliage , because the terrestrial environment is `` stickier '' than the oceans , greatly reducing the number of hops these chemical will experience .
	manualset3
118590	5	403865	13	NULL	NULL	0	NULL	terrestrial environment	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , no lag is predicted for less water soluble multihoppers ( K ( AW ) ) 1 ) , which are more likely to distribute into soils and foliage , because the terrestrial environment is `` stickier '' than the oceans , greatly reducing the number of hops these chemical will experience .
	manualset3
118591	6	403865	13	NULL	NULL	0	NULL	oceans	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , no lag is predicted for less water soluble multihoppers ( K ( AW ) ) 1 ) , which are more likely to distribute into soils and foliage , because the terrestrial environment is `` stickier '' than the oceans , greatly reducing the number of hops these chemical will experience .
	manualset3
118592	7	403865	13	NULL	NULL	0	NULL	number of hops	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , no lag is predicted for less water soluble multihoppers ( K ( AW ) ) 1 ) , which are more likely to distribute into soils and foliage , because the terrestrial environment is `` stickier '' than the oceans , greatly reducing the number of hops these chemical will experience .
	manualset3
118593	8	403865	13	NULL	NULL	0	NULL	chemical 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , no lag is predicted for less water soluble multihoppers ( K ( AW ) ) 1 ) , which are more likely to distribute into soils and foliage , because the terrestrial environment is `` stickier '' than the oceans , greatly reducing the number of hops these chemical will experience .
	manualset3
118594	1	403866	13	NULL	NULL	0	NULL	effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , we found a possible modifying effect of patient 's body mass index ( BMI ) on tumor TP53 .
	manualset3
118595	2	403866	13	NULL	NULL	0	NULL	patient 's 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , we found a possible modifying effect of patient 's body mass index ( BMI ) on tumor TP53 .
	manualset3
118596	3	403866	13	NULL	NULL	0	NULL	body mass index ( BMI ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , we found a possible modifying effect of patient 's body mass index ( BMI ) on tumor TP53 .
	manualset3
118597	4	403866	13	NULL	NULL	0	NULL	tumor TP53	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , we found a possible modifying effect of patient 's body mass index ( BMI ) on tumor TP53 .
	manualset3
118598	1	403867	13	NULL	NULL	0	NULL	Notch	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Notch does not overtly affect cell cycle entry or progression of CD4 ( + ) T cells .
	manualset3
118599	2	403867	13	NULL	NULL	NULL	NULL	cell cycle entry	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Notch does not overtly affect cell cycle entry or progression of CD4 ( + ) T cells .
	manualset3
118600	3	403867	13	NULL	NULL	0	NULL	progression 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Notch does not overtly affect cell cycle entry or progression of CD4 ( + ) T cells .
	manualset3
118601	4	403867	13	NULL	NULL	0	NULL	CD4 ( + ) T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Notch does not overtly affect cell cycle entry or progression of CD4 ( + ) T cells .
	manualset3
118602	1	403868	13	NULL	NULL	0	NULL	Notch 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Notch has also been implicated as a regulator of myogenesis , although its precise function there has remained controversial .
	manualset3
118603	2	403868	13	NULL	NULL	0	NULL	regulator	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Notch has also been implicated as a regulator of myogenesis , although its precise function there has remained controversial .
	manualset3
118604	3	403868	13	NULL	NULL	0	NULL	myogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Notch has also been implicated as a regulator of myogenesis , although its precise function there has remained controversial .
	manualset3
118605	4	403868	13	NULL	NULL	0	NULL	function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Notch has also been implicated as a regulator of myogenesis , although its precise function there has remained controversial .
	manualset3
118606	1	403869	13	NULL	NULL	0	NULL	Notch signaling 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Notch signaling is involved in cell differentiation and patterning during morphogenesis .
	manualset3
118607	2	403869	13	NULL	NULL	0	NULL	cell differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Notch signaling is involved in cell differentiation and patterning during morphogenesis .
	manualset3
118608	3	403869	13	NULL	NULL	0	NULL	morphogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Notch signaling is involved in cell differentiation and patterning during morphogenesis .
	manualset3
118609	1	403870	13	NULL	NULL	0	NULL	Notes 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Notes of a Case of Separation of the Uterus from the Body by Laceration during Labor .
	manualset3
118610	2	403870	13	NULL	NULL	0	NULL	Case of Separation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Notes of a Case of Separation of the Uterus from the Body by Laceration during Labor .
	manualset3
118611	3	403870	13	NULL	NULL	0	NULL	Uterus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Notes of a Case of Separation of the Uterus from the Body by Laceration during Labor .
	manualset3
118612	4	403870	13	NULL	NULL	0	NULL	Body	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Notes of a Case of Separation of the Uterus from the Body by Laceration during Labor .
	manualset3
118613	5	403870	13	NULL	NULL	0	NULL	Laceration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Notes of a Case of Separation of the Uterus from the Body by Laceration during Labor .
	manualset3
118614	6	403870	13	NULL	NULL	0	NULL	Labor 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Notes of a Case of Separation of the Uterus from the Body by Laceration during Labor .
	manualset3
118615	1	403871	13	NULL	NULL	0	NULL	scaffold preparation protocol 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Noticeably , scaffold preparation protocol presented here allowed the structural integrity to be maintained even with high template content ( 95 % ) and can easily be extended toward other classes of electrospun polymer matrices for tissue engineering .
	manualset3
118616	2	403871	13	NULL	NULL	0	NULL	structural integrity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Noticeably , scaffold preparation protocol presented here allowed the structural integrity to be maintained even with high template content ( 95 % ) and can easily be extended toward other classes of electrospun polymer matrices for tissue engineering .
	manualset3
118617	3	403871	13	NULL	NULL	0	NULL	high template content 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Noticeably , scaffold preparation protocol presented here allowed the structural integrity to be maintained even with high template content ( 95 % ) and can easily be extended toward other classes of electrospun polymer matrices for tissue engineering .
	manualset3
118618	4	403871	13	NULL	NULL	0	NULL	95 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Noticeably , scaffold preparation protocol presented here allowed the structural integrity to be maintained even with high template content ( 95 % ) and can easily be extended toward other classes of electrospun polymer matrices for tissue engineering .
	manualset3
118619	5	403871	13	NULL	NULL	0	NULL	classes of electrospun polymer matrices	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Noticeably , scaffold preparation protocol presented here allowed the structural integrity to be maintained even with high template content ( 95 % ) and can easily be extended toward other classes of electrospun polymer matrices for tissue engineering .
	manualset3
118620	6	403871	13	NULL	NULL	0	NULL	tissue engineering	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Noticeably , scaffold preparation protocol presented here allowed the structural integrity to be maintained even with high template content ( 95 % ) and can easily be extended toward other classes of electrospun polymer matrices for tissue engineering .
	manualset3
118621	1	403872	13	NULL	NULL	0	NULL	trial 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A controlled trial of glycopyrronium and l-hyoscyamine in the long-term treatment of duodenal ulcer .
	manualset3
118622	2	403872	13	NULL	NULL	0	NULL	glycopyrronium	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A controlled trial of glycopyrronium and l-hyoscyamine in the long-term treatment of duodenal ulcer .
	manualset3
118623	3	403872	13	NULL	NULL	0	NULL	l-hyoscyamine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A controlled trial of glycopyrronium and l-hyoscyamine in the long-term treatment of duodenal ulcer .
	manualset3
118624	4	403872	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A controlled trial of glycopyrronium and l-hyoscyamine in the long-term treatment of duodenal ulcer .
	manualset3
118625	5	403872	13	NULL	NULL	0	NULL	duodenal ulcer	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A controlled trial of glycopyrronium and l-hyoscyamine in the long-term treatment of duodenal ulcer .
	manualset3
118626	1	403873	13	NULL	NULL	0	NULL	chronic stress 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Noting that chronic stress or abuse in childhood can impair development of the brain region involved in learning and memory , the authors show how the extreme stress of being placed in an orphanage leads to abnormal brain development and decreased cognitive functioning .
	manualset3
118627	2	403873	13	NULL	NULL	0	NULL	abuse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Noting that chronic stress or abuse in childhood can impair development of the brain region involved in learning and memory , the authors show how the extreme stress of being placed in an orphanage leads to abnormal brain development and decreased cognitive functioning .
	manualset3
118628	3	403873	13	NULL	NULL	0	NULL	childhood 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Noting that chronic stress or abuse in childhood can impair development of the brain region involved in learning and memory , the authors show how the extreme stress of being placed in an orphanage leads to abnormal brain development and decreased cognitive functioning .
	manualset3
118629	4	403873	13	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Noting that chronic stress or abuse in childhood can impair development of the brain region involved in learning and memory , the authors show how the extreme stress of being placed in an orphanage leads to abnormal brain development and decreased cognitive functioning .
	manualset3
118630	5	403873	13	NULL	NULL	0	NULL	brain region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Noting that chronic stress or abuse in childhood can impair development of the brain region involved in learning and memory , the authors show how the extreme stress of being placed in an orphanage leads to abnormal brain development and decreased cognitive functioning .
	manualset3
118631	6	403873	13	NULL	NULL	0	NULL	learning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Noting that chronic stress or abuse in childhood can impair development of the brain region involved in learning and memory , the authors show how the extreme stress of being placed in an orphanage leads to abnormal brain development and decreased cognitive functioning .
	manualset3
118632	7	403873	13	NULL	NULL	0	NULL	memory	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Noting that chronic stress or abuse in childhood can impair development of the brain region involved in learning and memory , the authors show how the extreme stress of being placed in an orphanage leads to abnormal brain development and decreased cognitive functioning .
	manualset3
118633	8	403873	13	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Noting that chronic stress or abuse in childhood can impair development of the brain region involved in learning and memory , the authors show how the extreme stress of being placed in an orphanage leads to abnormal brain development and decreased cognitive functioning .
	manualset3
118634	9	403873	13	NULL	NULL	0	NULL	extreme stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Noting that chronic stress or abuse in childhood can impair development of the brain region involved in learning and memory , the authors show how the extreme stress of being placed in an orphanage leads to abnormal brain development and decreased cognitive functioning .
	manualset3
118635	10	403873	13	NULL	NULL	0	NULL	orphanage	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Noting that chronic stress or abuse in childhood can impair development of the brain region involved in learning and memory , the authors show how the extreme stress of being placed in an orphanage leads to abnormal brain development and decreased cognitive functioning .
	manualset3
118636	11	403873	13	NULL	NULL	0	NULL	abnormal brain development	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Noting that chronic stress or abuse in childhood can impair development of the brain region involved in learning and memory , the authors show how the extreme stress of being placed in an orphanage leads to abnormal brain development and decreased cognitive functioning .
	manualset3
118637	12	403873	13	NULL	NULL	0	NULL	cognitive functioning	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Noting that chronic stress or abuse in childhood can impair development of the brain region involved in learning and memory , the authors show how the extreme stress of being placed in an orphanage leads to abnormal brain development and decreased cognitive functioning .
	manualset3
118638	1	403874	13	NULL	NULL	0	NULL	gradual transitions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Notwithstanding gradual transitions between carcinoma in situ on the one hand and dysplasias and invasive cancer on the other hand , its histological separation from the latter is feasible in the uterine portio .
	manualset3
118639	2	403874	13	NULL	NULL	0	NULL	carcinoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Notwithstanding gradual transitions between carcinoma in situ on the one hand and dysplasias and invasive cancer on the other hand , its histological separation from the latter is feasible in the uterine portio .
	manualset3
118640	3	403874	13	NULL	NULL	0	NULL	dysplasias	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Notwithstanding gradual transitions between carcinoma in situ on the one hand and dysplasias and invasive cancer on the other hand , its histological separation from the latter is feasible in the uterine portio .
	manualset3
118641	4	403874	13	NULL	NULL	0	NULL	invasive cancer 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Notwithstanding gradual transitions between carcinoma in situ on the one hand and dysplasias and invasive cancer on the other hand , its histological separation from the latter is feasible in the uterine portio .
	manualset3
118642	5	403874	13	NULL	NULL	0	NULL	histological separation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Notwithstanding gradual transitions between carcinoma in situ on the one hand and dysplasias and invasive cancer on the other hand , its histological separation from the latter is feasible in the uterine portio .
	manualset3
118643	6	403874	13	NULL	NULL	0	NULL	latter 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Notwithstanding gradual transitions between carcinoma in situ on the one hand and dysplasias and invasive cancer on the other hand , its histological separation from the latter is feasible in the uterine portio .
	manualset3
118644	7	403874	13	NULL	NULL	0	NULL	uterine portio	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Notwithstanding gradual transitions between carcinoma in situ on the one hand and dysplasias and invasive cancer on the other hand , its histological separation from the latter is feasible in the uterine portio .
	manualset3
118645	1	403875	13	NULL	NULL	0	NULL	Nouns	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nouns and verbs in the brain : a review of behavioural , electrophysiological , neuropsychological and imaging studies .
	manualset3
118646	2	403875	13	NULL	NULL	0	NULL	verbs 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nouns and verbs in the brain : a review of behavioural , electrophysiological , neuropsychological and imaging studies .
	manualset3
118647	3	403875	13	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Nouns and verbs in the brain : a review of behavioural , electrophysiological , neuropsychological and imaging studies .
	manualset3
118648	4	403875	13	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Nouns and verbs in the brain : a review of behavioural , electrophysiological , neuropsychological and imaging studies .
	manualset3
118649	5	403875	13	NULL	NULL	0	NULL	behavioural studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nouns and verbs in the brain : a review of behavioural , electrophysiological , neuropsychological and imaging studies .
	manualset3
118650	6	403875	13	NULL	NULL	0	NULL	 electrophysiological studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nouns and verbs in the brain : a review of behavioural , electrophysiological , neuropsychological and imaging studies .
	manualset3
118651	7	403875	13	NULL	NULL	0	NULL	neuropsychological studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nouns and verbs in the brain : a review of behavioural , electrophysiological , neuropsychological and imaging studies .
	manualset3
118652	8	403875	13	NULL	NULL	0	NULL	imaging studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nouns and verbs in the brain : a review of behavioural , electrophysiological , neuropsychological and imaging studies .
	manualset3
118653	1	403876	13	NULL	NULL	0	NULL	Novel 5 ' - norcarbocyclic adenine analog	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel 5 ' - norcarbocyclic adenine and guanine phosphonic acid analogs with 6 ' , 6 ' - difluorine moiety were designed and synthesized from commercially available epichlorohydrin 5 .
	manualset3
118654	2	403876	13	NULL	NULL	0	NULL	guanine phosphonic acid analog	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel 5 ' - norcarbocyclic adenine and guanine phosphonic acid analogs with 6 ' , 6 ' - difluorine moiety were designed and synthesized from commercially available epichlorohydrin 5 .
	manualset3
118655	3	403876	13	NULL	NULL	0	NULL	 6 ' , 6 ' - difluorine moiety 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel 5 ' - norcarbocyclic adenine and guanine phosphonic acid analogs with 6 ' , 6 ' - difluorine moiety were designed and synthesized from commercially available epichlorohydrin 5 .
	manualset3
118656	4	403876	13	NULL	NULL	0	NULL	epichlorohydrin 5	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel 5 ' - norcarbocyclic adenine and guanine phosphonic acid analogs with 6 ' , 6 ' - difluorine moiety were designed and synthesized from commercially available epichlorohydrin 5 .
	manualset3
118657	1	403877	13	NULL	NULL	0	NULL	Novel application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel application of Phi29 DNA polymerase : RNA detection and analysis in vitro and in situ by target RNA-primed RCA .
	manualset3
118658	2	403877	13	NULL	NULL	0	NULL	Phi29 DNA polymerase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel application of Phi29 DNA polymerase : RNA detection and analysis in vitro and in situ by target RNA-primed RCA .
	manualset3
118659	3	403877	13	NULL	NULL	0	NULL	RNA detection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel application of Phi29 DNA polymerase : RNA detection and analysis in vitro and in situ by target RNA-primed RCA .
	manualset3
118660	4	403877	13	NULL	NULL	NULL	NULL	RNA analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Novel application of Phi29 DNA polymerase : RNA detection and analysis in vitro and in situ by target RNA-primed RCA .
	manualset3
118661	5	403877	13	NULL	NULL	0	NULL	target RNA-primed RCA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel application of Phi29 DNA polymerase : RNA detection and analysis in vitro and in situ by target RNA-primed RCA .
	manualset3
118662	1	403878	13	NULL	NULL	0	NULL	Novel blood pressure-related peptide hormones 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel blood pressure-related peptide hormones vying for prime time .
	manualset3
118663	2	403878	13	NULL	NULL	0	NULL	prime time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel blood pressure-related peptide hormones vying for prime time .
	manualset3
118664	1	403879	13	NULL	NULL	0	NULL	Novel calpain inhibitors 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel calpain inhibitors derived from phenyl alanine aldehydes or ketoamides carrying a benzoyl residue were prepared and evaluated for their biological potency .
	manualset3
118665	2	403879	13	NULL	NULL	0	NULL	phenyl alanine aldehydes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel calpain inhibitors derived from phenyl alanine aldehydes or ketoamides carrying a benzoyl residue were prepared and evaluated for their biological potency .
	manualset3
118666	3	403879	13	NULL	NULL	0	NULL	ketoamides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel calpain inhibitors derived from phenyl alanine aldehydes or ketoamides carrying a benzoyl residue were prepared and evaluated for their biological potency .
	manualset3
118667	4	403879	13	NULL	NULL	0	NULL	benzoyl residue	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel calpain inhibitors derived from phenyl alanine aldehydes or ketoamides carrying a benzoyl residue were prepared and evaluated for their biological potency .
	manualset3
118668	5	403879	13	NULL	NULL	0	NULL	biological potency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel calpain inhibitors derived from phenyl alanine aldehydes or ketoamides carrying a benzoyl residue were prepared and evaluated for their biological potency .
	manualset3
118669	1	403880	13	NULL	NULL	0	NULL	Novel chitosan-polycaprolactone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel chitosan-polycaprolactone blends as potential scaffold and carrier for corneal endothelial transplantation .
	manualset3
118670	2	403880	13	NULL	NULL	0	NULL	potential scaffold	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel chitosan-polycaprolactone blends as potential scaffold and carrier for corneal endothelial transplantation .
	manualset3
118671	3	403880	13	NULL	NULL	0	NULL	carrier 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel chitosan-polycaprolactone blends as potential scaffold and carrier for corneal endothelial transplantation .
	manualset3
118672	4	403880	13	NULL	NULL	0	NULL	corneal endothelial transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel chitosan-polycaprolactone blends as potential scaffold and carrier for corneal endothelial transplantation .
	manualset3
118673	1	403881	13	NULL	NULL	0	NULL	Novel combination neo-adjuvant chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel combination neo-adjuvant chemotherapy has been introduced for T3 gastric cancer patients .
	manualset3
118674	2	403881	13	NULL	NULL	0	NULL	T3 gastric cancer patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel combination neo-adjuvant chemotherapy has been introduced for T3 gastric cancer patients .
	manualset3
118675	1	403882	13	NULL	NULL	0	NULL	human proximal tubule cell line 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel conditionally immortalized human proximal tubule cell line expressing functional influx and efflux transporters .
	manualset3
118676	2	403882	13	NULL	NULL	0	NULL	functional influx transporters	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel conditionally immortalized human proximal tubule cell line expressing functional influx and efflux transporters .
	manualset3
118677	3	403882	13	NULL	NULL	0	NULL	efflux transporters	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel conditionally immortalized human proximal tubule cell line expressing functional influx and efflux transporters .
	manualset3
118678	1	403883	13	NULL	NULL	0	NULL	convenience sample	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A convenience sample of 145 families presenting to an urban tertiary care children 's hospital was surveyed using a previously validated instrument to gather information on levels of preparedness and factors influencing preparedness .
	manualset3
118679	2	403883	13	NULL	NULL	0	NULL	145 families	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A convenience sample of 145 families presenting to an urban tertiary care children 's hospital was surveyed using a previously validated instrument to gather information on levels of preparedness and factors influencing preparedness .
	manualset3
118680	3	403883	13	NULL	NULL	0	NULL	urban tertiary care children 's hospital 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A convenience sample of 145 families presenting to an urban tertiary care children 's hospital was surveyed using a previously validated instrument to gather information on levels of preparedness and factors influencing preparedness .
	manualset3
118681	4	403883	13	NULL	NULL	0	NULL	instrument 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A convenience sample of 145 families presenting to an urban tertiary care children 's hospital was surveyed using a previously validated instrument to gather information on levels of preparedness and factors influencing preparedness .
	manualset3
118682	5	403883	13	NULL	NULL	0	NULL	information	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A convenience sample of 145 families presenting to an urban tertiary care children 's hospital was surveyed using a previously validated instrument to gather information on levels of preparedness and factors influencing preparedness .
	manualset3
118683	6	403883	13	NULL	NULL	0	NULL	levels of preparedness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A convenience sample of 145 families presenting to an urban tertiary care children 's hospital was surveyed using a previously validated instrument to gather information on levels of preparedness and factors influencing preparedness .
	manualset3
118684	7	403883	13	NULL	NULL	0	NULL	factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A convenience sample of 145 families presenting to an urban tertiary care children 's hospital was surveyed using a previously validated instrument to gather information on levels of preparedness and factors influencing preparedness .
	manualset3
118685	8	403883	13	NULL	NULL	0	NULL	preparedness 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A convenience sample of 145 families presenting to an urban tertiary care children 's hospital was surveyed using a previously validated instrument to gather information on levels of preparedness and factors influencing preparedness .
	manualset3
118686	1	403884	13	NULL	NULL	0	NULL	Novel domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel domains in the hnRNP G/RBMX protein with distinct roles in RNA binding and targeting nascent transcripts .
	manualset3
118687	2	403884	13	NULL	NULL	0	NULL	 hnRNP G/RBMX protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel domains in the hnRNP G/RBMX protein with distinct roles in RNA binding and targeting nascent transcripts .
	manualset3
118688	3	403884	13	NULL	NULL	0	NULL	roles	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel domains in the hnRNP G/RBMX protein with distinct roles in RNA binding and targeting nascent transcripts .
	manualset3
118689	4	403884	13	NULL	NULL	0	NULL	RNA binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel domains in the hnRNP G/RBMX protein with distinct roles in RNA binding and targeting nascent transcripts .
	manualset3
118690	5	403884	13	NULL	NULL	0	NULL	nascent transcripts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel domains in the hnRNP G/RBMX protein with distinct roles in RNA binding and targeting nascent transcripts .
	manualset3
118691	1	403885	13	NULL	NULL	0	NULL	Novel folded protein domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel folded protein domains generated by combinatorial shuffling of polypeptide segments .
	manualset3
118692	2	403885	13	NULL	NULL	0	NULL	combinatorial shuffling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel folded protein domains generated by combinatorial shuffling of polypeptide segments .
	manualset3
118693	3	403885	13	NULL	NULL	0	NULL	polypeptide segments 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel folded protein domains generated by combinatorial shuffling of polypeptide segments .
	manualset3
118694	1	403886	13	NULL	NULL	0	NULL	Novel inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel inhibitors of nitric oxide synthase with antioxidant properties .
	manualset3
118695	2	403886	13	NULL	NULL	0	NULL	nitric oxide synthase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel inhibitors of nitric oxide synthase with antioxidant properties .
	manualset3
118696	3	403886	13	NULL	NULL	0	NULL	antioxidant properties	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel inhibitors of nitric oxide synthase with antioxidant properties .
	manualset3
118697	1	403887	13	NULL	NULL	0	NULL	Novel macroarray-based method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel macroarray-based method of Corynebacterium diphtheriae genotyping : evaluation in a field study in Belarus .
	manualset3
118698	2	403887	13	NULL	NULL	0	NULL	Corynebacterium diphtheriae genotyping	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel macroarray-based method of Corynebacterium diphtheriae genotyping : evaluation in a field study in Belarus .
	manualset3
118699	3	403887	13	NULL	NULL	0	NULL	evaluation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel macroarray-based method of Corynebacterium diphtheriae genotyping : evaluation in a field study in Belarus .
	manualset3
118700	4	403887	13	NULL	NULL	0	NULL	 field study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel macroarray-based method of Corynebacterium diphtheriae genotyping : evaluation in a field study in Belarus .
	manualset3
118701	5	403887	13	NULL	NULL	0	NULL	Belarus	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel macroarray-based method of Corynebacterium diphtheriae genotyping : evaluation in a field study in Belarus .
	manualset3
118702	1	403888	13	NULL	NULL	0	NULL	Novel non-natural amino acids 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel non-natural amino acids carrying a dansyl fluorescent group were designed , synthesized , and incorporated into various positions of streptavidin by using a CGGG four-base codon in an Escherichia coli in vitro translation system .
	manualset3
118703	2	403888	13	NULL	NULL	0	NULL	dansyl fluorescent group 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel non-natural amino acids carrying a dansyl fluorescent group were designed , synthesized , and incorporated into various positions of streptavidin by using a CGGG four-base codon in an Escherichia coli in vitro translation system .
	manualset3
118704	3	403888	13	NULL	NULL	NULL	NULL	various positions	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Novel non-natural amino acids carrying a dansyl fluorescent group were designed , synthesized , and incorporated into various positions of streptavidin by using a CGGG four-base codon in an Escherichia coli in vitro translation system .
	manualset3
118705	4	403888	13	NULL	NULL	0	NULL	streptavidin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel non-natural amino acids carrying a dansyl fluorescent group were designed , synthesized , and incorporated into various positions of streptavidin by using a CGGG four-base codon in an Escherichia coli in vitro translation system .
	manualset3
118706	5	403888	13	NULL	NULL	0	NULL	CGGG four-base codon	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel non-natural amino acids carrying a dansyl fluorescent group were designed , synthesized , and incorporated into various positions of streptavidin by using a CGGG four-base codon in an Escherichia coli in vitro translation system .
	manualset3
118707	6	403888	13	NULL	NULL	0	NULL	Escherichia coli in vitro translation system 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel non-natural amino acids carrying a dansyl fluorescent group were designed , synthesized , and incorporated into various positions of streptavidin by using a CGGG four-base codon in an Escherichia coli in vitro translation system .
	manualset3
118708	1	403889	13	NULL	NULL	NULL	NULL	Novel pathway 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Novel pathway of toluene catabolism in the trichloroethylene-degrading bacterium g4 .
	manualset3
118709	2	403889	13	NULL	NULL	0	NULL	toluene catabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel pathway of toluene catabolism in the trichloroethylene-degrading bacterium g4 .
	manualset3
118710	3	403889	13	NULL	NULL	0	NULL	trichloroethylene-degrading bacterium g4	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel pathway of toluene catabolism in the trichloroethylene-degrading bacterium g4 .
	manualset3
118711	1	403890	13	NULL	NULL	0	NULL	Novel polyurethanes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel polyurethanes with interconnected porous structure induce in vivo tissue remodeling and accompanied vascularization .
	manualset3
118712	2	403890	13	NULL	NULL	0	NULL	porous structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel polyurethanes with interconnected porous structure induce in vivo tissue remodeling and accompanied vascularization .
	manualset3
118713	3	403890	13	NULL	NULL	0	NULL	tissue 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel polyurethanes with interconnected porous structure induce in vivo tissue remodeling and accompanied vascularization .
	manualset3
118714	4	403890	13	NULL	NULL	0	NULL	vascularization 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel polyurethanes with interconnected porous structure induce in vivo tissue remodeling and accompanied vascularization .
	manualset3
118715	1	403891	13	NULL	NULL	0	NULL	Novel pulsed regimens	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel pulsed regimens using alfacalcidol and calcitriol , while clearly effective , have not fulfilled initial high expectations of superiority in the context of comparative studies .
	manualset3
118716	2	403891	13	NULL	NULL	0	NULL	alfacalcidol 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel pulsed regimens using alfacalcidol and calcitriol , while clearly effective , have not fulfilled initial high expectations of superiority in the context of comparative studies .
	manualset3
118717	3	403891	13	NULL	NULL	0	NULL	calcitriol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel pulsed regimens using alfacalcidol and calcitriol , while clearly effective , have not fulfilled initial high expectations of superiority in the context of comparative studies .
	manualset3
118718	4	403891	13	NULL	NULL	0	NULL	expectations of superiority	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel pulsed regimens using alfacalcidol and calcitriol , while clearly effective , have not fulfilled initial high expectations of superiority in the context of comparative studies .
	manualset3
118719	5	403891	13	NULL	NULL	0	NULL	context	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel pulsed regimens using alfacalcidol and calcitriol , while clearly effective , have not fulfilled initial high expectations of superiority in the context of comparative studies .
	manualset3
118720	6	403891	13	NULL	NULL	0	NULL	comparative studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel pulsed regimens using alfacalcidol and calcitriol , while clearly effective , have not fulfilled initial high expectations of superiority in the context of comparative studies .
	manualset3
118721	1	403892	13	NULL	NULL	0	NULL	Novel techniques 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel techniques such as serum proteomics , microarrays , and metastatic cell isolation methods may better predict outcome in advanced prostate cancer .
	manualset3
118722	2	403892	13	NULL	NULL	0	NULL	serum proteomics	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel techniques such as serum proteomics , microarrays , and metastatic cell isolation methods may better predict outcome in advanced prostate cancer .
	manualset3
118723	3	403892	13	NULL	NULL	0	NULL	microarrays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel techniques such as serum proteomics , microarrays , and metastatic cell isolation methods may better predict outcome in advanced prostate cancer .
	manualset3
118724	4	403892	13	NULL	NULL	0	NULL	metastatic cell isolation methods 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel techniques such as serum proteomics , microarrays , and metastatic cell isolation methods may better predict outcome in advanced prostate cancer .
	manualset3
118725	5	403892	13	NULL	NULL	0	NULL	outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel techniques such as serum proteomics , microarrays , and metastatic cell isolation methods may better predict outcome in advanced prostate cancer .
	manualset3
118726	6	403892	13	NULL	NULL	0	NULL	prostate cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel techniques such as serum proteomics , microarrays , and metastatic cell isolation methods may better predict outcome in advanced prostate cancer .
	manualset3
118727	1	403893	13	NULL	NULL	0	NULL	reports 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Now , reports Caroline Richmond , another surge of litigation may be on the horizon because a 1996 change makes it possible for lawyers to take cases on a contingency basis .
	manualset3
118728	2	403893	13	NULL	NULL	0	NULL	Caroline Richmond	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Now , reports Caroline Richmond , another surge of litigation may be on the horizon because a 1996 change makes it possible for lawyers to take cases on a contingency basis .
	manualset3
118729	3	403893	13	NULL	NULL	0	NULL	surge of litigation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Now , reports Caroline Richmond , another surge of litigation may be on the horizon because a 1996 change makes it possible for lawyers to take cases on a contingency basis .
	manualset3
118730	4	403893	13	NULL	NULL	0	NULL	horizon	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Now , reports Caroline Richmond , another surge of litigation may be on the horizon because a 1996 change makes it possible for lawyers to take cases on a contingency basis .
	manualset3
118731	5	403893	13	NULL	NULL	0	NULL	1996	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Now , reports Caroline Richmond , another surge of litigation may be on the horizon because a 1996 change makes it possible for lawyers to take cases on a contingency basis .
	manualset3
118732	6	403893	13	NULL	NULL	0	NULL	change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Now , reports Caroline Richmond , another surge of litigation may be on the horizon because a 1996 change makes it possible for lawyers to take cases on a contingency basis .
	manualset3
118733	7	403893	13	NULL	NULL	0	NULL	lawyers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Now , reports Caroline Richmond , another surge of litigation may be on the horizon because a 1996 change makes it possible for lawyers to take cases on a contingency basis .
	manualset3
118734	8	403893	13	NULL	NULL	0	NULL	cases 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Now , reports Caroline Richmond , another surge of litigation may be on the horizon because a 1996 change makes it possible for lawyers to take cases on a contingency basis .
	manualset3
118735	9	403893	13	NULL	NULL	0	NULL	contingency basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Now , reports Caroline Richmond , another surge of litigation may be on the horizon because a 1996 change makes it possible for lawyers to take cases on a contingency basis .
	manualset3
118736	1	403894	13	NULL	NULL	0	NULL	climate changes	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Now , the climate changes systematically at a considerable speed due to global warming .
	manualset3
118737	2	403894	13	NULL	NULL	0	NULL	speed 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Now , the climate changes systematically at a considerable speed due to global warming .
	manualset3
121670	3	403894	13	NULL	NULL	0	NULL	global warming	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Now , the climate changes systematically at a considerable speed due to global warming .
	manualset3
118738	1	403895	13	NULL	NULL	0	NULL	acute exacerbation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Now it is the elderly who have an acute exacerbation of their peripheral vascular disease .
	manualset3
118739	2	403895	13	NULL	NULL	0	NULL	peripheral vascular disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Now it is the elderly who have an acute exacerbation of their peripheral vascular disease .
	manualset3
118740	1	403896	13	NULL	NULL	0	NULL	adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nowadays , it is recommended that adults need a minimum of 800-1 , 000 U/day when their exposure to the sun is inadequate ( in Poland from October to April ) .
	manualset3
118741	2	403896	13	NULL	NULL	0	NULL	minimum of 800-1 , 000 U/day	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Nowadays , it is recommended that adults need a minimum of 800-1 , 000 U/day when their exposure to the sun is inadequate ( in Poland from October to April ) .
	manualset3
118742	3	403896	13	NULL	NULL	0	NULL	exposure 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nowadays , it is recommended that adults need a minimum of 800-1 , 000 U/day when their exposure to the sun is inadequate ( in Poland from October to April ) .
	manualset3
118743	4	403896	13	NULL	NULL	0	NULL	sun	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Nowadays , it is recommended that adults need a minimum of 800-1 , 000 U/day when their exposure to the sun is inadequate ( in Poland from October to April ) .
	manualset3
118744	5	403896	13	NULL	NULL	0	NULL	Poland	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Nowadays , it is recommended that adults need a minimum of 800-1 , 000 U/day when their exposure to the sun is inadequate ( in Poland from October to April ) .
	manualset3
118745	6	403896	13	NULL	NULL	0	NULL	October to April	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Nowadays , it is recommended that adults need a minimum of 800-1 , 000 U/day when their exposure to the sun is inadequate ( in Poland from October to April ) .
	manualset3
118746	1	403897	13	NULL	NULL	0	NULL	Noxious mechanical stimuli 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Noxious mechanical stimuli , but not thermal stimuli , increased the release of immunoreactive substance P ( iSP ) .
	manualset3
118747	2	403897	13	NULL	NULL	0	NULL	thermal stimuli	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Noxious mechanical stimuli , but not thermal stimuli , increased the release of immunoreactive substance P ( iSP ) .
	manualset3
118748	3	403897	13	NULL	NULL	0	NULL	release 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Noxious mechanical stimuli , but not thermal stimuli , increased the release of immunoreactive substance P ( iSP ) .
	manualset3
118749	4	403897	13	NULL	NULL	0	NULL	immunoreactive substance P ( iSP )	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Noxious mechanical stimuli , but not thermal stimuli , increased the release of immunoreactive substance P ( iSP ) .
	manualset3
118750	1	403898	13	NULL	NULL	0	NULL	Noxious stimuli 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Noxious stimuli also excite a system with contralateral topographical projection , high synaptic security and termination in lamina IV .
	manualset3
118751	2	403898	13	NULL	NULL	0	NULL	system 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Noxious stimuli also excite a system with contralateral topographical projection , high synaptic security and termination in lamina IV .
	manualset3
118752	3	403898	13	NULL	NULL	0	NULL	contralateral topographical projection	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Noxious stimuli also excite a system with contralateral topographical projection , high synaptic security and termination in lamina IV .
	manualset3
118753	4	403898	13	NULL	NULL	0	NULL	synaptic security	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Noxious stimuli also excite a system with contralateral topographical projection , high synaptic security and termination in lamina IV .
	manualset3
118754	5	403898	13	NULL	NULL	0	NULL	termination 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Noxious stimuli also excite a system with contralateral topographical projection , high synaptic security and termination in lamina IV .
	manualset3
118755	6	403898	13	NULL	NULL	0	NULL	lamina IV	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Noxious stimuli also excite a system with contralateral topographical projection , high synaptic security and termination in lamina IV .
	manualset3
118756	1	403899	13	NULL	NULL	NULL	NULL	Nuclear area	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nuclear area and a roundness factor were studied by histomorphometry in 35 cases , and the DNA content was analyzed in 27 cases .
	manualset3
118757	2	403899	13	NULL	NULL	0	NULL	roundness factor	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear area and a roundness factor were studied by histomorphometry in 35 cases , and the DNA content was analyzed in 27 cases .
	manualset3
118758	3	403899	13	NULL	NULL	NULL	NULL	histomorphometry 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nuclear area and a roundness factor were studied by histomorphometry in 35 cases , and the DNA content was analyzed in 27 cases .
	manualset3
118759	4	403899	13	NULL	NULL	0	NULL	35 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear area and a roundness factor were studied by histomorphometry in 35 cases , and the DNA content was analyzed in 27 cases .
	manualset3
118760	5	403899	13	NULL	NULL	0	NULL	DNA content	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear area and a roundness factor were studied by histomorphometry in 35 cases , and the DNA content was analyzed in 27 cases .
	manualset3
118761	6	403899	13	NULL	NULL	0	NULL	27 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear area and a roundness factor were studied by histomorphometry in 35 cases , and the DNA content was analyzed in 27 cases .
	manualset3
118762	1	403900	13	NULL	NULL	0	NULL	rapid method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A convenient , rapid method for the resolution of enantiomeric amino acids using chiral phases on stainless-steel capillary gas chromatographic columns .
	manualset3
118763	2	403900	13	NULL	NULL	0	NULL	resolution 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A convenient , rapid method for the resolution of enantiomeric amino acids using chiral phases on stainless-steel capillary gas chromatographic columns .
	manualset3
118764	3	403900	13	NULL	NULL	0	NULL	enantiomeric amino acids 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A convenient , rapid method for the resolution of enantiomeric amino acids using chiral phases on stainless-steel capillary gas chromatographic columns .
	manualset3
118765	4	403900	13	NULL	NULL	0	NULL	chiral phases	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A convenient , rapid method for the resolution of enantiomeric amino acids using chiral phases on stainless-steel capillary gas chromatographic columns .
	manualset3
118766	5	403900	13	NULL	NULL	0	NULL	stainless-steel capillary gas chromatographic columns	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A convenient , rapid method for the resolution of enantiomeric amino acids using chiral phases on stainless-steel capillary gas chromatographic columns .
	manualset3
118767	1	403901	13	NULL	NULL	0	NULL	Nuclear factor erythroid-derived 2-like 2 ( Nrf2 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear factor erythroid-derived 2-like 2 ( Nrf2 ) controls the expression of several enzymes that are protective against oxidative stress .
	manualset3
118768	2	403901	13	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear factor erythroid-derived 2-like 2 ( Nrf2 ) controls the expression of several enzymes that are protective against oxidative stress .
	manualset3
118769	3	403901	13	NULL	NULL	0	NULL	several enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear factor erythroid-derived 2-like 2 ( Nrf2 ) controls the expression of several enzymes that are protective against oxidative stress .
	manualset3
118770	4	403901	13	NULL	NULL	0	NULL	oxidative stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear factor erythroid-derived 2-like 2 ( Nrf2 ) controls the expression of several enzymes that are protective against oxidative stress .
	manualset3
118771	1	403902	13	NULL	NULL	0	NULL	Nuclear proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear proteins isolated from enterocytes showed increased binding of the HNF-1 alpha complex with a concomitant decrease in the HNF-1 beta-containing complex to the SIF3 element both during the suckling-weaning developmental transition and Caco-2 cell differentiation .
	manualset3
118772	2	403902	13	NULL	NULL	0	NULL	enterocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear proteins isolated from enterocytes showed increased binding of the HNF-1 alpha complex with a concomitant decrease in the HNF-1 beta-containing complex to the SIF3 element both during the suckling-weaning developmental transition and Caco-2 cell differentiation .
	manualset3
118773	3	403902	13	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear proteins isolated from enterocytes showed increased binding of the HNF-1 alpha complex with a concomitant decrease in the HNF-1 beta-containing complex to the SIF3 element both during the suckling-weaning developmental transition and Caco-2 cell differentiation .
	manualset3
118774	4	403902	13	NULL	NULL	NULL	NULL	HNF-1 alpha complex	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nuclear proteins isolated from enterocytes showed increased binding of the HNF-1 alpha complex with a concomitant decrease in the HNF-1 beta-containing complex to the SIF3 element both during the suckling-weaning developmental transition and Caco-2 cell differentiation .
	manualset3
118776	6	403902	13	NULL	NULL	0	NULL	decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear proteins isolated from enterocytes showed increased binding of the HNF-1 alpha complex with a concomitant decrease in the HNF-1 beta-containing complex to the SIF3 element both during the suckling-weaning developmental transition and Caco-2 cell differentiation .
	manualset3
118777	7	403902	13	NULL	NULL	0	NULL	HNF-1 beta-containing complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear proteins isolated from enterocytes showed increased binding of the HNF-1 alpha complex with a concomitant decrease in the HNF-1 beta-containing complex to the SIF3 element both during the suckling-weaning developmental transition and Caco-2 cell differentiation .
	manualset3
118778	8	403902	13	NULL	NULL	0	NULL	SIF3 element 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear proteins isolated from enterocytes showed increased binding of the HNF-1 alpha complex with a concomitant decrease in the HNF-1 beta-containing complex to the SIF3 element both during the suckling-weaning developmental transition and Caco-2 cell differentiation .
	manualset3
118779	9	403902	13	NULL	NULL	0	NULL	developmental transition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear proteins isolated from enterocytes showed increased binding of the HNF-1 alpha complex with a concomitant decrease in the HNF-1 beta-containing complex to the SIF3 element both during the suckling-weaning developmental transition and Caco-2 cell differentiation .
	manualset3
118780	10	403902	13	NULL	NULL	0	NULL	Caco-2 cell 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear proteins isolated from enterocytes showed increased binding of the HNF-1 alpha complex with a concomitant decrease in the HNF-1 beta-containing complex to the SIF3 element both during the suckling-weaning developmental transition and Caco-2 cell differentiation .
	manualset3
118781	11	403902	13	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear proteins isolated from enterocytes showed increased binding of the HNF-1 alpha complex with a concomitant decrease in the HNF-1 beta-containing complex to the SIF3 element both during the suckling-weaning developmental transition and Caco-2 cell differentiation .
	manualset3
118782	1	403903	13	NULL	NULL	0	NULL	Nuclear ribonucleoprotein complexes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear ribonucleoprotein complexes containing U1 and U2 RNA .
	manualset3
118783	2	403903	13	NULL	NULL	0	NULL	U1 RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear ribonucleoprotein complexes containing U1 and U2 RNA .
	manualset3
118784	3	403903	13	NULL	NULL	0	NULL	U2 RNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear ribonucleoprotein complexes containing U1 and U2 RNA .
	manualset3
118785	1	403904	13	NULL	NULL	0	NULL	Nuclear run-on analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear run-on analysis showed that phorbol ester induced the transcription of interleukin 1 beta but did not induce it in the presence of cycloheximide .
	manualset3
118786	2	403904	13	NULL	NULL	0	NULL	phorbol ester 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear run-on analysis showed that phorbol ester induced the transcription of interleukin 1 beta but did not induce it in the presence of cycloheximide .
	manualset3
118787	3	403904	13	NULL	NULL	0	NULL	transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear run-on analysis showed that phorbol ester induced the transcription of interleukin 1 beta but did not induce it in the presence of cycloheximide .
	manualset3
118788	4	403904	13	NULL	NULL	0	NULL	interleukin 1 beta	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear run-on analysis showed that phorbol ester induced the transcription of interleukin 1 beta but did not induce it in the presence of cycloheximide .
	manualset3
118789	5	403904	13	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear run-on analysis showed that phorbol ester induced the transcription of interleukin 1 beta but did not induce it in the presence of cycloheximide .
	manualset3
118790	6	403904	13	NULL	NULL	0	NULL	cycloheximide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear run-on analysis showed that phorbol ester induced the transcription of interleukin 1 beta but did not induce it in the presence of cycloheximide .
	manualset3
118791	1	403905	13	NULL	NULL	0	NULL	Nuclear tau	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear tau immunoreactivity in presenile dementia with motor neuron disease : a case report .
	manualset3
118792	2	403905	13	NULL	NULL	0	NULL	immunoreactivity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear tau immunoreactivity in presenile dementia with motor neuron disease : a case report .
	manualset3
118793	3	403905	13	NULL	NULL	0	NULL	presenile dementia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear tau immunoreactivity in presenile dementia with motor neuron disease : a case report .
	manualset3
118794	4	403905	13	NULL	NULL	0	NULL	motor neuron disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear tau immunoreactivity in presenile dementia with motor neuron disease : a case report .
	manualset3
118795	5	403905	13	NULL	NULL	0	NULL	case report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear tau immunoreactivity in presenile dementia with motor neuron disease : a case report .
	manualset3
118796	1	403906	13	NULL	NULL	0	NULL	Nuclear terrorism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear terrorism : health and environmental hazards and threats from ionizing and nuclear radiation .
	manualset3
118797	2	403906	13	NULL	NULL	0	NULL	health hazards 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear terrorism : health and environmental hazards and threats from ionizing and nuclear radiation .
	manualset3
118798	3	403906	13	NULL	NULL	0	NULL	environmental hazards 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear terrorism : health and environmental hazards and threats from ionizing and nuclear radiation .
	manualset3
118799	4	403906	13	NULL	NULL	0	NULL	threats	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear terrorism : health and environmental hazards and threats from ionizing and nuclear radiation .
	manualset3
118800	5	403906	13	NULL	NULL	0	NULL	nuclear radiation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear terrorism : health and environmental hazards and threats from ionizing and nuclear radiation .
	manualset3
118801	1	403907	13	NULL	NULL	0	NULL	Nuclear transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear transcription and actinomycin D chase experiments indicated that VTs stabilize labile preproET-1 mRNA transcripts in endothelial cells .
	manualset3
118802	2	403907	13	NULL	NULL	0	NULL	actinomycin D chase experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear transcription and actinomycin D chase experiments indicated that VTs stabilize labile preproET-1 mRNA transcripts in endothelial cells .
	manualset3
118803	3	403907	13	NULL	NULL	0	NULL	VTs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear transcription and actinomycin D chase experiments indicated that VTs stabilize labile preproET-1 mRNA transcripts in endothelial cells .
	manualset3
118804	4	403907	13	NULL	NULL	0	NULL	preproET-1 mRNA transcripts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear transcription and actinomycin D chase experiments indicated that VTs stabilize labile preproET-1 mRNA transcripts in endothelial cells .
	manualset3
118805	5	403907	13	NULL	NULL	0	NULL	endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclear transcription and actinomycin D chase experiments indicated that VTs stabilize labile preproET-1 mRNA transcripts in endothelial cells .
	manualset3
118806	1	403908	13	NULL	NULL	0	NULL	Nucleic acid sequence analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleic acid sequence analysis showed that the divergent clones code for a protein lacking a 26-amino acid NH2-terminal putative membrane-spanning signal peptide .
	manualset3
118807	2	403908	13	NULL	NULL	0	NULL	clones	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleic acid sequence analysis showed that the divergent clones code for a protein lacking a 26-amino acid NH2-terminal putative membrane-spanning signal peptide .
	manualset3
118808	3	403908	13	NULL	NULL	0	NULL	code 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleic acid sequence analysis showed that the divergent clones code for a protein lacking a 26-amino acid NH2-terminal putative membrane-spanning signal peptide .
	manualset3
118809	4	403908	13	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleic acid sequence analysis showed that the divergent clones code for a protein lacking a 26-amino acid NH2-terminal putative membrane-spanning signal peptide .
	manualset3
118810	5	403908	13	NULL	NULL	0	NULL	26-amino acid NH2-terminal putative membrane-spanning signal peptide 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleic acid sequence analysis showed that the divergent clones code for a protein lacking a 26-amino acid NH2-terminal putative membrane-spanning signal peptide .
	manualset3
118811	1	403909	13	NULL	NULL	0	NULL	Nucleoli	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleoli are prominent subnuclear organelles , and are known to be hubs of ribosome synthesis .
	manualset3
118812	2	403909	13	NULL	NULL	0	NULL	subnuclear organelles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleoli are prominent subnuclear organelles , and are known to be hubs of ribosome synthesis .
	manualset3
118813	3	403909	13	NULL	NULL	0	NULL	hubs	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleoli are prominent subnuclear organelles , and are known to be hubs of ribosome synthesis .
	manualset3
118814	4	403909	13	NULL	NULL	0	NULL	ribosome synthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleoli are prominent subnuclear organelles , and are known to be hubs of ribosome synthesis .
	manualset3
118815	1	403910	13	NULL	NULL	0	NULL	Nucleosomal peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleosomal peptides in histone regions H2B ( 10-33 ) , H4 ( 16-39 ) ( and overlapping H4 ( 14-28 ) ) , H4 ( 71-94 ) , and H3 ( 91-105 ) ( and overlapping H3 ( 100-114 ) ) were recurrently recognized by CD4 T cells from the patients with lupus .
	manualset3
118816	2	403910	13	NULL	NULL	0	NULL	histone regions 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleosomal peptides in histone regions H2B ( 10-33 ) , H4 ( 16-39 ) ( and overlapping H4 ( 14-28 ) ) , H4 ( 71-94 ) , and H3 ( 91-105 ) ( and overlapping H3 ( 100-114 ) ) were recurrently recognized by CD4 T cells from the patients with lupus .
	manualset3
118817	3	403910	13	NULL	NULL	0	NULL	H2B ( 10-33 )	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleosomal peptides in histone regions H2B ( 10-33 ) , H4 ( 16-39 ) ( and overlapping H4 ( 14-28 ) ) , H4 ( 71-94 ) , and H3 ( 91-105 ) ( and overlapping H3 ( 100-114 ) ) were recurrently recognized by CD4 T cells from the patients with lupus .
	manualset3
118818	4	403910	13	NULL	NULL	0	NULL	H4 ( 16-39 ) 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleosomal peptides in histone regions H2B ( 10-33 ) , H4 ( 16-39 ) ( and overlapping H4 ( 14-28 ) ) , H4 ( 71-94 ) , and H3 ( 91-105 ) ( and overlapping H3 ( 100-114 ) ) were recurrently recognized by CD4 T cells from the patients with lupus .
	manualset3
118819	5	403910	13	NULL	NULL	0	NULL	H4 ( 14-28 )	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleosomal peptides in histone regions H2B ( 10-33 ) , H4 ( 16-39 ) ( and overlapping H4 ( 14-28 ) ) , H4 ( 71-94 ) , and H3 ( 91-105 ) ( and overlapping H3 ( 100-114 ) ) were recurrently recognized by CD4 T cells from the patients with lupus .
	manualset3
118820	6	403910	13	NULL	NULL	0	NULL	H4 ( 71-94 )	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleosomal peptides in histone regions H2B ( 10-33 ) , H4 ( 16-39 ) ( and overlapping H4 ( 14-28 ) ) , H4 ( 71-94 ) , and H3 ( 91-105 ) ( and overlapping H3 ( 100-114 ) ) were recurrently recognized by CD4 T cells from the patients with lupus .
	manualset3
118821	7	403910	13	NULL	NULL	0	NULL	H3 ( 91-105 )	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleosomal peptides in histone regions H2B ( 10-33 ) , H4 ( 16-39 ) ( and overlapping H4 ( 14-28 ) ) , H4 ( 71-94 ) , and H3 ( 91-105 ) ( and overlapping H3 ( 100-114 ) ) were recurrently recognized by CD4 T cells from the patients with lupus .
	manualset3
118822	8	403910	13	NULL	NULL	0	NULL	H3 ( 100-114 )	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleosomal peptides in histone regions H2B ( 10-33 ) , H4 ( 16-39 ) ( and overlapping H4 ( 14-28 ) ) , H4 ( 71-94 ) , and H3 ( 91-105 ) ( and overlapping H3 ( 100-114 ) ) were recurrently recognized by CD4 T cells from the patients with lupus .
	manualset3
118823	9	403910	13	NULL	NULL	0	NULL	CD4 T cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleosomal peptides in histone regions H2B ( 10-33 ) , H4 ( 16-39 ) ( and overlapping H4 ( 14-28 ) ) , H4 ( 71-94 ) , and H3 ( 91-105 ) ( and overlapping H3 ( 100-114 ) ) were recurrently recognized by CD4 T cells from the patients with lupus .
	manualset3
118824	10	403910	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleosomal peptides in histone regions H2B ( 10-33 ) , H4 ( 16-39 ) ( and overlapping H4 ( 14-28 ) ) , H4 ( 71-94 ) , and H3 ( 91-105 ) ( and overlapping H3 ( 100-114 ) ) were recurrently recognized by CD4 T cells from the patients with lupus .
	manualset3
118825	11	403910	13	NULL	NULL	0	NULL	lupus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleosomal peptides in histone regions H2B ( 10-33 ) , H4 ( 16-39 ) ( and overlapping H4 ( 14-28 ) ) , H4 ( 71-94 ) , and H3 ( 91-105 ) ( and overlapping H3 ( 100-114 ) ) were recurrently recognized by CD4 T cells from the patients with lupus .
	manualset3
118826	1	403911	13	NULL	NULL	0	NULL	Nucleosome assembly proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleosome assembly proteins play important roles in chromatin remodeling , which determines gene expression , cell proliferation and terminal differentiation .
	manualset3
118827	2	403911	13	NULL	NULL	0	NULL	roles 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleosome assembly proteins play important roles in chromatin remodeling , which determines gene expression , cell proliferation and terminal differentiation .
	manualset3
118828	3	403911	13	NULL	NULL	0	NULL	chromatin remodeling	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleosome assembly proteins play important roles in chromatin remodeling , which determines gene expression , cell proliferation and terminal differentiation .
	manualset3
118829	4	403911	13	NULL	NULL	0	NULL	gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleosome assembly proteins play important roles in chromatin remodeling , which determines gene expression , cell proliferation and terminal differentiation .
	manualset3
118830	5	403911	13	NULL	NULL	0	NULL	cell proliferation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleosome assembly proteins play important roles in chromatin remodeling , which determines gene expression , cell proliferation and terminal differentiation .
	manualset3
118831	6	403911	13	NULL	NULL	0	NULL	terminal differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleosome assembly proteins play important roles in chromatin remodeling , which determines gene expression , cell proliferation and terminal differentiation .
	manualset3
118832	1	403912	13	NULL	NULL	0	NULL	Nucleotide sequence of cDNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleotide sequence of cDNA encoding beta-luffin , another ribosome-inactivating protein from Luffa cylindrica .
	manualset3
118833	2	403912	13	NULL	NULL	0	NULL	beta-luffin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleotide sequence of cDNA encoding beta-luffin , another ribosome-inactivating protein from Luffa cylindrica .
	manualset3
118834	3	403912	13	NULL	NULL	0	NULL	ribosome-inactivating protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleotide sequence of cDNA encoding beta-luffin , another ribosome-inactivating protein from Luffa cylindrica .
	manualset3
118835	4	403912	13	NULL	NULL	0	NULL	Luffa cylindrica	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Nucleotide sequence of cDNA encoding beta-luffin , another ribosome-inactivating protein from Luffa cylindrica .
	manualset3
118836	1	403913	13	NULL	NULL	0	NULL	Null mutants 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Null mutants also fail to express CEH-10 , suggesting that CEH-10 regulates its own expression .
	manualset3
118837	2	403913	13	NULL	NULL	0	NULL	CEH-10 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Null mutants also fail to express CEH-10 , suggesting that CEH-10 regulates its own expression .
	manualset3
118838	3	403913	13	NULL	NULL	0	NULL	CEH-10	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Null mutants also fail to express CEH-10 , suggesting that CEH-10 regulates its own expression .
	manualset3
118839	4	403913	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Null mutants also fail to express CEH-10 , suggesting that CEH-10 regulates its own expression .
	manualset3
118840	1	403914	13	NULL	NULL	0	NULL	Numbers	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Numbers of CD4 + and CD8 + cells were also lower in infected , irradiated mice .
	manualset3
118841	2	403914	13	NULL	NULL	0	NULL	CD4 + cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Numbers of CD4 + and CD8 + cells were also lower in infected , irradiated mice .
	manualset3
118842	3	403914	13	NULL	NULL	0	NULL	CD8 + cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Numbers of CD4 + and CD8 + cells were also lower in infected , irradiated mice .
	manualset3
118843	4	403914	13	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Numbers of CD4 + and CD8 + cells were also lower in infected , irradiated mice .
	manualset3
118844	1	403915	13	NULL	NULL	0	NULL	synthesis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A convenient synthesis of 7-halo-1-indanones and 8-halo-1-tetralones .
	manualset3
118845	2	403915	13	NULL	NULL	0	NULL	7-halo-1-indanones	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A convenient synthesis of 7-halo-1-indanones and 8-halo-1-tetralones .
	manualset3
118846	3	403915	13	NULL	NULL	0	NULL	8-halo-1-tetralones	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A convenient synthesis of 7-halo-1-indanones and 8-halo-1-tetralones .
	manualset3
118847	1	403916	13	NULL	NULL	0	NULL	GAST-like genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous GAST-like genes have been identified in various plant species .
	manualset3
118848	2	403916	13	NULL	NULL	0	NULL	various plant species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous GAST-like genes have been identified in various plant species .
	manualset3
118849	1	403917	13	NULL	NULL	0	NULL	Numerous cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous cells with the appearance of microglia were found to constitutively express class I MHC antigens , while only rare cells expressed class II ( Ia ) antigens .
	manualset3
118850	2	403917	13	NULL	NULL	0	NULL	appearance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous cells with the appearance of microglia were found to constitutively express class I MHC antigens , while only rare cells expressed class II ( Ia ) antigens .
	manualset3
118851	3	403917	13	NULL	NULL	0	NULL	microglia 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous cells with the appearance of microglia were found to constitutively express class I MHC antigens , while only rare cells expressed class II ( Ia ) antigens .
	manualset3
118852	4	403917	13	NULL	NULL	0	NULL	class I MHC antigens	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous cells with the appearance of microglia were found to constitutively express class I MHC antigens , while only rare cells expressed class II ( Ia ) antigens .
	manualset3
118853	5	403917	13	NULL	NULL	0	NULL	rare cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous cells with the appearance of microglia were found to constitutively express class I MHC antigens , while only rare cells expressed class II ( Ia ) antigens .
	manualset3
118854	6	403917	13	NULL	NULL	0	NULL	class II ( Ia ) antigens	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous cells with the appearance of microglia were found to constitutively express class I MHC antigens , while only rare cells expressed class II ( Ia ) antigens .
	manualset3
118855	1	403918	13	NULL	NULL	0	NULL	Numerous non-cardiovascular effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous non-cardiovascular effects of pet ownership have been reported , largely in the psychosocial domain , but the relationship is complex and can vary with demographic and social factors .
	manualset3
118856	2	403918	13	NULL	NULL	0	NULL	pet ownership 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous non-cardiovascular effects of pet ownership have been reported , largely in the psychosocial domain , but the relationship is complex and can vary with demographic and social factors .
	manualset3
118857	3	403918	13	NULL	NULL	0	NULL	psychosocial domain	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous non-cardiovascular effects of pet ownership have been reported , largely in the psychosocial domain , but the relationship is complex and can vary with demographic and social factors .
	manualset3
118858	4	403918	13	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous non-cardiovascular effects of pet ownership have been reported , largely in the psychosocial domain , but the relationship is complex and can vary with demographic and social factors .
	manualset3
118859	5	403918	13	NULL	NULL	0	NULL	demographic factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous non-cardiovascular effects of pet ownership have been reported , largely in the psychosocial domain , but the relationship is complex and can vary with demographic and social factors .
	manualset3
118860	6	403918	13	NULL	NULL	0	NULL	social factors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous non-cardiovascular effects of pet ownership have been reported , largely in the psychosocial domain , but the relationship is complex and can vary with demographic and social factors .
	manualset3
118861	1	403919	13	NULL	NULL	0	NULL	antiangiogenic compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous potentially useful antiangiogenic compounds are in development ; two drugs are presently in clinical trials for treatment of the preproliferative stage of PDR , while two are in clinical trials for treatment of ME .
	manualset3
118862	2	403919	13	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous potentially useful antiangiogenic compounds are in development ; two drugs are presently in clinical trials for treatment of the preproliferative stage of PDR , while two are in clinical trials for treatment of ME .
	manualset3
118863	3	403919	13	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous potentially useful antiangiogenic compounds are in development ; two drugs are presently in clinical trials for treatment of the preproliferative stage of PDR , while two are in clinical trials for treatment of ME .
	manualset3
118864	4	403919	13	NULL	NULL	0	NULL	drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous potentially useful antiangiogenic compounds are in development ; two drugs are presently in clinical trials for treatment of the preproliferative stage of PDR , while two are in clinical trials for treatment of ME .
	manualset3
118865	5	403919	13	NULL	NULL	0	NULL	clinical trials 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous potentially useful antiangiogenic compounds are in development ; two drugs are presently in clinical trials for treatment of the preproliferative stage of PDR , while two are in clinical trials for treatment of ME .
	manualset3
118866	6	403919	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous potentially useful antiangiogenic compounds are in development ; two drugs are presently in clinical trials for treatment of the preproliferative stage of PDR , while two are in clinical trials for treatment of ME .
	manualset3
118867	7	403919	13	NULL	NULL	0	NULL	preproliferative stage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous potentially useful antiangiogenic compounds are in development ; two drugs are presently in clinical trials for treatment of the preproliferative stage of PDR , while two are in clinical trials for treatment of ME .
	manualset3
118868	8	403919	13	NULL	NULL	0	NULL	PDR	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous potentially useful antiangiogenic compounds are in development ; two drugs are presently in clinical trials for treatment of the preproliferative stage of PDR , while two are in clinical trials for treatment of ME .
	manualset3
118869	9	403919	13	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous potentially useful antiangiogenic compounds are in development ; two drugs are presently in clinical trials for treatment of the preproliferative stage of PDR , while two are in clinical trials for treatment of ME .
	manualset3
118870	10	403919	13	NULL	NULL	0	NULL	clinical trials	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous potentially useful antiangiogenic compounds are in development ; two drugs are presently in clinical trials for treatment of the preproliferative stage of PDR , while two are in clinical trials for treatment of ME .
	manualset3
118871	11	403919	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous potentially useful antiangiogenic compounds are in development ; two drugs are presently in clinical trials for treatment of the preproliferative stage of PDR , while two are in clinical trials for treatment of ME .
	manualset3
118872	12	403919	13	NULL	NULL	0	NULL	ME 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous potentially useful antiangiogenic compounds are in development ; two drugs are presently in clinical trials for treatment of the preproliferative stage of PDR , while two are in clinical trials for treatment of ME .
	manualset3
118873	1	403920	13	NULL	NULL	0	NULL	Numerous studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous studies report that adverse levels of cardiovascular diseases risk factors are associated with adiposity in children .
	manualset3
118874	2	403920	13	NULL	NULL	0	NULL	adverse levels 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous studies report that adverse levels of cardiovascular diseases risk factors are associated with adiposity in children .
	manualset3
118875	3	403920	13	NULL	NULL	NULL	NULL	cardiovascular diseases  	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Numerous studies report that adverse levels of cardiovascular diseases risk factors are associated with adiposity in children .
	manualset3
118876	4	403920	13	NULL	NULL	0	NULL	adiposity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous studies report that adverse levels of cardiovascular diseases risk factors are associated with adiposity in children .
	manualset3
118877	5	403920	13	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous studies report that adverse levels of cardiovascular diseases risk factors are associated with adiposity in children .
	manualset3
118878	6	403920	13	NULL	NULL	0	NULL	risk factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Numerous studies report that adverse levels of cardiovascular diseases risk factors are associated with adiposity in children .
	manualset3
118879	1	403921	13	NULL	NULL	0	NULL	Nurse	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurse retention : is it worth it ?
	manualset3
118880	2	403921	13	NULL	NULL	0	NULL	retention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurse retention : is it worth it ?
	manualset3
118881	1	403922	13	NULL	NULL	0	NULL	Nurse titration clinics	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurse titration clinics to achieve rapid control of blood pressure .
	manualset3
118882	2	403922	13	NULL	NULL	0	NULL	control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurse titration clinics to achieve rapid control of blood pressure .
	manualset3
118883	3	403922	13	NULL	NULL	0	NULL	blood pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurse titration clinics to achieve rapid control of blood pressure .
	manualset3
118884	1	403923	13	NULL	NULL	0	NULL	Nurse practitioners	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurse practitioners : stretching the limits of nursing practice .
	manualset3
118885	2	403923	13	NULL	NULL	0	NULL	limits	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurse practitioners : stretching the limits of nursing practice .
	manualset3
118886	3	403923	13	NULL	NULL	0	NULL	nursing practice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurse practitioners : stretching the limits of nursing practice .
	manualset3
118887	1	403924	13	NULL	NULL	0	NULL	Nurse case management 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurse case management for the frail elderly : a curriculum to prepare nurses for that role .
	manualset3
118888	2	403924	13	NULL	NULL	0	NULL	curriculum	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurse case management for the frail elderly : a curriculum to prepare nurses for that role .
	manualset3
118889	3	403924	13	NULL	NULL	0	NULL	nurses	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurse case management for the frail elderly : a curriculum to prepare nurses for that role .
	manualset3
118890	4	403924	13	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurse case management for the frail elderly : a curriculum to prepare nurses for that role .
	manualset3
118891	1	403925	13	NULL	NULL	0	NULL	Nurses	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurses can seize the opportunity to offer smoking interventions .
	manualset3
118892	2	403925	13	NULL	NULL	0	NULL	opportunity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurses can seize the opportunity to offer smoking interventions .
	manualset3
118893	3	403925	13	NULL	NULL	0	NULL	interventions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurses can seize the opportunity to offer smoking interventions .
	manualset3
118894	1	403926	13	NULL	NULL	0	NULL	Nursing informatics 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Nursing informatics is a growing field with many opportunities for nursing involvement .
	manualset3
118895	2	403926	13	NULL	NULL	0	NULL	 field	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Nursing informatics is a growing field with many opportunities for nursing involvement .
	manualset3
118896	3	403926	13	NULL	NULL	0	NULL	opportunities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nursing informatics is a growing field with many opportunities for nursing involvement .
	manualset3
118897	4	403926	13	NULL	NULL	0	NULL	involvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nursing informatics is a growing field with many opportunities for nursing involvement .
	manualset3
118898	1	403927	13	NULL	NULL	0	NULL	Nursing care study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nursing care study : anorexia nervosa .
	manualset3
118899	2	403927	13	NULL	NULL	0	NULL	anorexia nervosa	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nursing care study : anorexia nervosa .
	manualset3
118900	1	403928	13	NULL	NULL	0	NULL	Nursing ethics 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Nursing ethics : understanding the moral life .
	manualset3
118901	2	403928	13	NULL	NULL	0	NULL	moral life	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nursing ethics : understanding the moral life .
	manualset3
118902	1	403929	13	NULL	NULL	0	NULL	Nursing students	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nursing students assisted clients through the cold clinic 's five stations , establishing relationships and practicing communication and assessment skills .
	manualset3
118903	2	403929	13	NULL	NULL	0	NULL	clients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nursing students assisted clients through the cold clinic 's five stations , establishing relationships and practicing communication and assessment skills .
	manualset3
118904	3	403929	13	NULL	NULL	0	NULL	cold clinic 's five stations	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Nursing students assisted clients through the cold clinic 's five stations , establishing relationships and practicing communication and assessment skills .
	manualset3
118905	4	403929	13	NULL	NULL	0	NULL	relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Nursing students assisted clients through the cold clinic 's five stations , establishing relationships and practicing communication and assessment skills .
	manualset3
118906	5	403929	13	NULL	NULL	0	NULL	communication	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nursing students assisted clients through the cold clinic 's five stations , establishing relationships and practicing communication and assessment skills .
	manualset3
118907	6	403929	13	NULL	NULL	0	NULL	assessment skills 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Nursing students assisted clients through the cold clinic 's five stations , establishing relationships and practicing communication and assessment skills .
	manualset3
118908	1	403930	13	NULL	NULL	0	NULL	Nutritional value	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Nutritional value of milk and meat products derived from cloning .
	manualset3
118909	2	403930	13	NULL	NULL	0	NULL	milk 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Nutritional value of milk and meat products derived from cloning .
	manualset3
118910	3	403930	13	NULL	NULL	0	NULL	meat products 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Nutritional value of milk and meat products derived from cloning .
	manualset3
121676	4	403930	13	NULL	NULL	0	NULL	cloning	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nutritional value of milk and meat products derived from cloning .
	manualset3
118912	1	403931	13	NULL	NULL	0	NULL	Nylon-6 capillary-channeled polymer ( C-CP ) fibers 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Nylon-6 capillary-channeled polymer ( C-CP ) fibers are used as the stationary phase for the hydrophobic interaction chromatography ( HIC ) separation of a synthetic protein mixture composed of ribonuclease A , lysozyme , and holotransferrin .
	manualset3
118913	2	403931	13	NULL	NULL	NULL	NULL	stationary phase	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nylon-6 capillary-channeled polymer ( C-CP ) fibers are used as the stationary phase for the hydrophobic interaction chromatography ( HIC ) separation of a synthetic protein mixture composed of ribonuclease A , lysozyme , and holotransferrin .
	manualset3
118914	3	403931	13	NULL	NULL	0	NULL	hydrophobic interaction chromatography ( HIC )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nylon-6 capillary-channeled polymer ( C-CP ) fibers are used as the stationary phase for the hydrophobic interaction chromatography ( HIC ) separation of a synthetic protein mixture composed of ribonuclease A , lysozyme , and holotransferrin .
	manualset3
118915	4	403931	13	NULL	NULL	0	NULL	separation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nylon-6 capillary-channeled polymer ( C-CP ) fibers are used as the stationary phase for the hydrophobic interaction chromatography ( HIC ) separation of a synthetic protein mixture composed of ribonuclease A , lysozyme , and holotransferrin .
	manualset3
118916	5	403931	13	NULL	NULL	0	NULL	synthetic protein mixture 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nylon-6 capillary-channeled polymer ( C-CP ) fibers are used as the stationary phase for the hydrophobic interaction chromatography ( HIC ) separation of a synthetic protein mixture composed of ribonuclease A , lysozyme , and holotransferrin .
	manualset3
118917	6	403931	13	NULL	NULL	0	NULL	ribonuclease A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nylon-6 capillary-channeled polymer ( C-CP ) fibers are used as the stationary phase for the hydrophobic interaction chromatography ( HIC ) separation of a synthetic protein mixture composed of ribonuclease A , lysozyme , and holotransferrin .
	manualset3
118918	7	403931	13	NULL	NULL	0	NULL	lysozyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nylon-6 capillary-channeled polymer ( C-CP ) fibers are used as the stationary phase for the hydrophobic interaction chromatography ( HIC ) separation of a synthetic protein mixture composed of ribonuclease A , lysozyme , and holotransferrin .
	manualset3
118919	8	403931	13	NULL	NULL	0	NULL	holotransferrin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nylon-6 capillary-channeled polymer ( C-CP ) fibers are used as the stationary phase for the hydrophobic interaction chromatography ( HIC ) separation of a synthetic protein mixture composed of ribonuclease A , lysozyme , and holotransferrin .
	manualset3
118920	1	403932	13	NULL	NULL	0	NULL	Nymphs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Nymphs were placed within an arena containing a humidity gradient ranging from 45 to 95 % relative humidity ( RH ) .
	manualset3
118921	2	403932	13	NULL	NULL	0	NULL	arena	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Nymphs were placed within an arena containing a humidity gradient ranging from 45 to 95 % relative humidity ( RH ) .
	manualset3
118922	3	403932	13	NULL	NULL	0	NULL	humidity gradient	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Nymphs were placed within an arena containing a humidity gradient ranging from 45 to 95 % relative humidity ( RH ) .
	manualset3
118923	4	403932	13	NULL	NULL	0	NULL	 45 to 95 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Nymphs were placed within an arena containing a humidity gradient ranging from 45 to 95 % relative humidity ( RH ) .
	manualset3
118924	5	403932	13	NULL	NULL	0	NULL	relative humidity ( RH ) 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Nymphs were placed within an arena containing a humidity gradient ranging from 45 to 95 % relative humidity ( RH ) .
	manualset3
118925	1	403933	13	NULL	NULL	0	NULL	O2 consumption	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	O2 consumption , heart rate and subjective ratings under conditions of relaxation and active coping .
	manualset3
118926	2	403933	13	NULL	NULL	0	NULL	heart rate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	O2 consumption , heart rate and subjective ratings under conditions of relaxation and active coping .
	manualset3
118927	3	403933	13	NULL	NULL	0	NULL	subjective ratings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	O2 consumption , heart rate and subjective ratings under conditions of relaxation and active coping .
	manualset3
118928	4	403933	13	NULL	NULL	0	NULL	conditions of relaxation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	O2 consumption , heart rate and subjective ratings under conditions of relaxation and active coping .
	manualset3
118929	5	403933	13	NULL	NULL	0	NULL	active coping	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	O2 consumption , heart rate and subjective ratings under conditions of relaxation and active coping .
	manualset3
118930	1	403934	13	NULL	NULL	0	NULL	O6-meG levels 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	O6-meG levels increased during the treatment period , peaking at 11.1 + / - 1.25 micromol/mol dG in PBMCs and at 4.25 + / - 0.79 micromol/mol dG in tumor biopsies .
	manualset3
118931	2	403934	13	NULL	NULL	0	NULL	treatment period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	O6-meG levels increased during the treatment period , peaking at 11.1 + / - 1.25 micromol/mol dG in PBMCs and at 4.25 + / - 0.79 micromol/mol dG in tumor biopsies .
	manualset3
118932	3	403934	13	NULL	NULL	0	NULL	11.1 + / - 1.25 micromol/mol dG 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	O6-meG levels increased during the treatment period , peaking at 11.1 + / - 1.25 micromol/mol dG in PBMCs and at 4.25 + / - 0.79 micromol/mol dG in tumor biopsies .
	manualset3
118933	4	403934	13	NULL	NULL	0	NULL	PBMCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	O6-meG levels increased during the treatment period , peaking at 11.1 + / - 1.25 micromol/mol dG in PBMCs and at 4.25 + / - 0.79 micromol/mol dG in tumor biopsies .
	manualset3
118934	5	403934	13	NULL	NULL	0	NULL	tumor biopsies	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	O6-meG levels increased during the treatment period , peaking at 11.1 + / - 1.25 micromol/mol dG in PBMCs and at 4.25 + / - 0.79 micromol/mol dG in tumor biopsies .
	manualset3
118935	6	403934	13	NULL	NULL	0	NULL	4.25 + / - 0.79 micromol/mol dG	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	O6-meG levels increased during the treatment period , peaking at 11.1 + / - 1.25 micromol/mol dG in PBMCs and at 4.25 + / - 0.79 micromol/mol dG in tumor biopsies .
	manualset3
118936	1	403935	13	NULL	NULL	0	NULL	O6-methylguanine-DNA methyltransferase ( MGMT ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	O6-methylguanine-DNA methyltransferase ( MGMT ) , a ubiquitous DNA repair protein , removes the mutagenic DNA adduct O6-alkylguanine , which is synthesized both endogenously and after exposure to alkylnitrosamines and alkylating antitumor drugs such as 2-chloroethyl-N-nitrosourea ( CNU ) .
	manualset3
118937	2	403935	13	NULL	NULL	0	NULL	ubiquitous DNA repair protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	O6-methylguanine-DNA methyltransferase ( MGMT ) , a ubiquitous DNA repair protein , removes the mutagenic DNA adduct O6-alkylguanine , which is synthesized both endogenously and after exposure to alkylnitrosamines and alkylating antitumor drugs such as 2-chloroethyl-N-nitrosourea ( CNU ) .
	manualset3
118938	3	403935	13	NULL	NULL	0	NULL	mutagenic DNA adduct O6-alkylguanine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	O6-methylguanine-DNA methyltransferase ( MGMT ) , a ubiquitous DNA repair protein , removes the mutagenic DNA adduct O6-alkylguanine , which is synthesized both endogenously and after exposure to alkylnitrosamines and alkylating antitumor drugs such as 2-chloroethyl-N-nitrosourea ( CNU ) .
	manualset3
118939	4	403935	13	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	O6-methylguanine-DNA methyltransferase ( MGMT ) , a ubiquitous DNA repair protein , removes the mutagenic DNA adduct O6-alkylguanine , which is synthesized both endogenously and after exposure to alkylnitrosamines and alkylating antitumor drugs such as 2-chloroethyl-N-nitrosourea ( CNU ) .
	manualset3
118940	5	403935	13	NULL	NULL	0	NULL	alkylnitrosamines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	O6-methylguanine-DNA methyltransferase ( MGMT ) , a ubiquitous DNA repair protein , removes the mutagenic DNA adduct O6-alkylguanine , which is synthesized both endogenously and after exposure to alkylnitrosamines and alkylating antitumor drugs such as 2-chloroethyl-N-nitrosourea ( CNU ) .
	manualset3
118941	6	403935	13	NULL	NULL	0	NULL	alkylating antitumor drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	O6-methylguanine-DNA methyltransferase ( MGMT ) , a ubiquitous DNA repair protein , removes the mutagenic DNA adduct O6-alkylguanine , which is synthesized both endogenously and after exposure to alkylnitrosamines and alkylating antitumor drugs such as 2-chloroethyl-N-nitrosourea ( CNU ) .
	manualset3
118942	7	403935	13	NULL	NULL	0	NULL	2-chloroethyl-N-nitrosourea ( CNU ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	O6-methylguanine-DNA methyltransferase ( MGMT ) , a ubiquitous DNA repair protein , removes the mutagenic DNA adduct O6-alkylguanine , which is synthesized both endogenously and after exposure to alkylnitrosamines and alkylating antitumor drugs such as 2-chloroethyl-N-nitrosourea ( CNU ) .
	manualset3
118943	1	403936	13	NULL	NULL	0	NULL	prevention program	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A coordinated prevention program which included research and a variety of educational efforts , has been underway for the past five years .
	manualset3
118944	2	403936	13	NULL	NULL	0	NULL	research 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A coordinated prevention program which included research and a variety of educational efforts , has been underway for the past five years .
	manualset3
118946	3	403936	13	NULL	NULL	0	NULL	variety of educational efforts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A coordinated prevention program which included research and a variety of educational efforts , has been underway for the past five years .
	manualset3
118947	4	403936	13	NULL	NULL	0	NULL	past five years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A coordinated prevention program which included research and a variety of educational efforts , has been underway for the past five years .
	manualset3
118948	1	403937	13	NULL	NULL	0	NULL	O7-LPS-deficient mutants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	O7-LPS-deficient mutants of VW187 were complemented with pJHCV31 and pJHCV32 , confirming that these cosmids contain genetic information that is essential for the expression of the O7 polysaccharide .
	manualset3
118949	2	403937	13	NULL	NULL	0	NULL	VW187	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	O7-LPS-deficient mutants of VW187 were complemented with pJHCV31 and pJHCV32 , confirming that these cosmids contain genetic information that is essential for the expression of the O7 polysaccharide .
	manualset3
118950	3	403937	13	NULL	NULL	0	NULL	pJHCV31	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	O7-LPS-deficient mutants of VW187 were complemented with pJHCV31 and pJHCV32 , confirming that these cosmids contain genetic information that is essential for the expression of the O7 polysaccharide .
	manualset3
118951	4	403937	13	NULL	NULL	0	NULL	pJHCV32	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	O7-LPS-deficient mutants of VW187 were complemented with pJHCV31 and pJHCV32 , confirming that these cosmids contain genetic information that is essential for the expression of the O7 polysaccharide .
	manualset3
118952	5	403937	13	NULL	NULL	0	NULL	cosmids	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	O7-LPS-deficient mutants of VW187 were complemented with pJHCV31 and pJHCV32 , confirming that these cosmids contain genetic information that is essential for the expression of the O7 polysaccharide .
	manualset3
118953	6	403937	13	NULL	NULL	0	NULL	genetic information	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	O7-LPS-deficient mutants of VW187 were complemented with pJHCV31 and pJHCV32 , confirming that these cosmids contain genetic information that is essential for the expression of the O7 polysaccharide .
	manualset3
118954	7	403937	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	O7-LPS-deficient mutants of VW187 were complemented with pJHCV31 and pJHCV32 , confirming that these cosmids contain genetic information that is essential for the expression of the O7 polysaccharide .
	manualset3
118955	8	403937	13	NULL	NULL	0	NULL	O7 polysaccharide	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	O7-LPS-deficient mutants of VW187 were complemented with pJHCV31 and pJHCV32 , confirming that these cosmids contain genetic information that is essential for the expression of the O7 polysaccharide .
	manualset3
118956	1	403938	13	NULL	NULL	0	NULL	OA-exposed animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	OA-exposed animals developed OA-specific IgG1 antibodies , AHR and airway eosinophilia ( sham/OA , RSV/OA and RSV6/OA groups .
	manualset3
118957	2	403938	13	NULL	NULL	0	NULL	OA-specific IgG1 antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	OA-exposed animals developed OA-specific IgG1 antibodies , AHR and airway eosinophilia ( sham/OA , RSV/OA and RSV6/OA groups .
	manualset3
118958	3	403938	13	NULL	NULL	0	NULL	AHR	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	OA-exposed animals developed OA-specific IgG1 antibodies , AHR and airway eosinophilia ( sham/OA , RSV/OA and RSV6/OA groups .
	manualset3
118959	4	403938	13	NULL	NULL	0	NULL	airway eosinophilia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	OA-exposed animals developed OA-specific IgG1 antibodies , AHR and airway eosinophilia ( sham/OA , RSV/OA and RSV6/OA groups .
	manualset3
118960	5	403938	13	NULL	NULL	0	NULL	sham/OA groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	OA-exposed animals developed OA-specific IgG1 antibodies , AHR and airway eosinophilia ( sham/OA , RSV/OA and RSV6/OA groups .
	manualset3
118961	6	403938	13	NULL	NULL	0	NULL	RSV/OA groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	OA-exposed animals developed OA-specific IgG1 antibodies , AHR and airway eosinophilia ( sham/OA , RSV/OA and RSV6/OA groups .
	manualset3
118962	7	403938	13	NULL	NULL	0	NULL	RSV6/OA groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	OA-exposed animals developed OA-specific IgG1 antibodies , AHR and airway eosinophilia ( sham/OA , RSV/OA and RSV6/OA groups .
	manualset3
118963	1	403939	13	NULL	NULL	0	NULL	OA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	OA caused significant increases in tau phosphorylation confirming that tau is a substrate for PP2A in endothelium .
	manualset3
118964	2	403939	13	NULL	NULL	0	NULL	increases	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	OA caused significant increases in tau phosphorylation confirming that tau is a substrate for PP2A in endothelium .
	manualset3
118965	3	403939	13	NULL	NULL	0	NULL	tau 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	OA caused significant increases in tau phosphorylation confirming that tau is a substrate for PP2A in endothelium .
	manualset3
118966	4	403939	13	NULL	NULL	0	NULL	phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	OA caused significant increases in tau phosphorylation confirming that tau is a substrate for PP2A in endothelium .
	manualset3
118967	5	403939	13	NULL	NULL	0	NULL	tau 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	OA caused significant increases in tau phosphorylation confirming that tau is a substrate for PP2A in endothelium .
	manualset3
118968	6	403939	13	NULL	NULL	0	NULL	substrate	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	OA caused significant increases in tau phosphorylation confirming that tau is a substrate for PP2A in endothelium .
	manualset3
118969	7	403939	13	NULL	NULL	0	NULL	PP2A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	OA caused significant increases in tau phosphorylation confirming that tau is a substrate for PP2A in endothelium .
	manualset3
118970	8	403939	13	NULL	NULL	0	NULL	endothelium	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	OA caused significant increases in tau phosphorylation confirming that tau is a substrate for PP2A in endothelium .
	manualset3
118971	1	403940	13	NULL	NULL	0	NULL	purpose	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	OBJECTIVE : The purpose of this study was to examine the reference sound pressure level ( RSPL ) for Korean speech audiometry which was defined as the reference speech recognition threshold level ( RSRTL ) equivalent to 0 dB HL at the audiometer .
	manualset3
118972	2	403940	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	OBJECTIVE : The purpose of this study was to examine the reference sound pressure level ( RSPL ) for Korean speech audiometry which was defined as the reference speech recognition threshold level ( RSRTL ) equivalent to 0 dB HL at the audiometer .
	manualset3
118973	3	403940	13	NULL	NULL	0	NULL	reference sound pressure level ( RSPL )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	OBJECTIVE : The purpose of this study was to examine the reference sound pressure level ( RSPL ) for Korean speech audiometry which was defined as the reference speech recognition threshold level ( RSRTL ) equivalent to 0 dB HL at the audiometer .
	manualset3
118974	4	403940	13	NULL	NULL	0	NULL	Korean speech audiometry	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	OBJECTIVE : The purpose of this study was to examine the reference sound pressure level ( RSPL ) for Korean speech audiometry which was defined as the reference speech recognition threshold level ( RSRTL ) equivalent to 0 dB HL at the audiometer .
	manualset3
118975	5	403940	13	NULL	NULL	0	NULL	reference speech recognition threshold level ( RSRTL )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	OBJECTIVE : The purpose of this study was to examine the reference sound pressure level ( RSPL ) for Korean speech audiometry which was defined as the reference speech recognition threshold level ( RSRTL ) equivalent to 0 dB HL at the audiometer .
	manualset3
118977	7	403940	13	NULL	NULL	0	NULL	 0 dB HL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	OBJECTIVE : The purpose of this study was to examine the reference sound pressure level ( RSPL ) for Korean speech audiometry which was defined as the reference speech recognition threshold level ( RSRTL ) equivalent to 0 dB HL at the audiometer .
	manualset3
118978	8	403940	13	NULL	NULL	0	NULL	audiometer	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	OBJECTIVE : The purpose of this study was to examine the reference sound pressure level ( RSPL ) for Korean speech audiometry which was defined as the reference speech recognition threshold level ( RSRTL ) equivalent to 0 dB HL at the audiometer .
	manualset3
118979	1	403941	13	NULL	NULL	0	NULL	Diabetes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	OBJECTIVE Diabetes and hypertension often co-occur and share risk factors .
	manualset3
118980	2	403941	13	NULL	NULL	0	NULL	hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	OBJECTIVE Diabetes and hypertension often co-occur and share risk factors .
	manualset3
118982	4	403941	13	NULL	NULL	0	NULL	risk factors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	OBJECTIVE Diabetes and hypertension often co-occur and share risk factors .
	manualset3
118983	1	403942	13	NULL	NULL	0	NULL	OBSERVATIONS	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	OBSERVATIONS ON THE FORMATION OF WHEALS : IV .
	manualset3
118984	2	403942	13	NULL	NULL	0	NULL	FORMATION	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	OBSERVATIONS ON THE FORMATION OF WHEALS : IV .
	manualset3
118985	3	403942	13	NULL	NULL	0	NULL	WHEALS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	OBSERVATIONS ON THE FORMATION OF WHEALS : IV .
	manualset3
118986	1	403943	13	NULL	NULL	0	NULL	OC	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	OC of the skull base was diagnosed , with possibly a concurrent lesion of the condyle .
	manualset3
118987	2	403943	13	NULL	NULL	0	NULL	skull base	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	OC of the skull base was diagnosed , with possibly a concurrent lesion of the condyle .
	manualset3
118988	3	403943	13	NULL	NULL	0	NULL	lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	OC of the skull base was diagnosed , with possibly a concurrent lesion of the condyle .
	manualset3
118989	4	403943	13	NULL	NULL	0	NULL	condyle	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	OC of the skull base was diagnosed , with possibly a concurrent lesion of the condyle .
	manualset3
118990	1	403944	13	NULL	NULL	0	NULL	OECs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	OECs appear to regulate molecules of the extracellular matrix ( ECM ) that inhibit axonal growth .
	manualset3
118991	2	403944	13	NULL	NULL	0	NULL	molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	OECs appear to regulate molecules of the extracellular matrix ( ECM ) that inhibit axonal growth .
	manualset3
118992	3	403944	13	NULL	NULL	0	NULL	extracellular matrix ( ECM )	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	OECs appear to regulate molecules of the extracellular matrix ( ECM ) that inhibit axonal growth .
	manualset3
118993	4	403944	13	NULL	NULL	0	NULL	axonal growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	OECs appear to regulate molecules of the extracellular matrix ( ECM ) that inhibit axonal growth .
	manualset3
118994	1	403945	13	NULL	NULL	0	NULL	OH 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	OH , the ultimate toxic species , via the metal-catalyzed Fenton reaction .
	manualset3
118995	2	403945	13	NULL	NULL	0	NULL	toxic species	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	OH , the ultimate toxic species , via the metal-catalyzed Fenton reaction .
	manualset3
118996	3	403945	13	NULL	NULL	0	NULL	metal-catalyzed Fenton reaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	OH , the ultimate toxic species , via the metal-catalyzed Fenton reaction .
	manualset3
119177	1	403946	13	NULL	NULL	0	NULL	OKA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	OKA did not affect glycogen synthesis in denervated muscle except for abolishing a small insulin effect .
	manualset3
119178	2	403946	13	NULL	NULL	0	NULL	glycogen synthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	OKA did not affect glycogen synthesis in denervated muscle except for abolishing a small insulin effect .
	manualset3
119179	3	403946	13	NULL	NULL	0	NULL	muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	OKA did not affect glycogen synthesis in denervated muscle except for abolishing a small insulin effect .
	manualset3
119181	4	403946	13	NULL	NULL	NULL	NULL	insulin effect	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	OKA did not affect glycogen synthesis in denervated muscle except for abolishing a small insulin effect .
	manualset3
119182	1	403947	13	NULL	NULL	0	NULL	correlation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A correlation also existed in diabetics between fucosyl - ( but not sialyl - ) transferase activity and glycosylated serum protein ( r = 0.52 , p less than 0.001 ) .
	manualset3
119183	2	403947	13	NULL	NULL	0	NULL	diabetics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A correlation also existed in diabetics between fucosyl - ( but not sialyl - ) transferase activity and glycosylated serum protein ( r = 0.52 , p less than 0.001 ) .
	manualset3
119184	3	403947	13	NULL	NULL	0	NULL	fucosyl - ( but not sialyl - ) transferase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A correlation also existed in diabetics between fucosyl - ( but not sialyl - ) transferase activity and glycosylated serum protein ( r = 0.52 , p less than 0.001 ) .
	manualset3
119185	4	403947	13	NULL	NULL	0	NULL	glycosylated serum protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A correlation also existed in diabetics between fucosyl - ( but not sialyl - ) transferase activity and glycosylated serum protein ( r = 0.52 , p less than 0.001 ) .
	manualset3
119186	5	403947	13	NULL	NULL	0	NULL	 r = 0.52 , p less than 0.001 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A correlation also existed in diabetics between fucosyl - ( but not sialyl - ) transferase activity and glycosylated serum protein ( r = 0.52 , p less than 0.001 ) .
	manualset3
119187	1	403948	13	NULL	NULL	0	NULL	OTC	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	OTC is a cysteine precursor required for the synthesis of glutathione , an important antioxidant .
	manualset3
119188	2	403948	13	NULL	NULL	0	NULL	cysteine precursor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	OTC is a cysteine precursor required for the synthesis of glutathione , an important antioxidant .
	manualset3
119189	3	403948	13	NULL	NULL	0	NULL	synthesis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	OTC is a cysteine precursor required for the synthesis of glutathione , an important antioxidant .
	manualset3
119190	4	403948	13	NULL	NULL	0	NULL	antioxidant	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	OTC is a cysteine precursor required for the synthesis of glutathione , an important antioxidant .
	manualset3
119191	5	403948	13	NULL	NULL	0	NULL	glutathione	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	OTC is a cysteine precursor required for the synthesis of glutathione , an important antioxidant .
	manualset3
119192	1	403949	13	NULL	NULL	0	NULL	Obese children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Obese children tended to have high CRP levels , BP elevation , and slight dyslipidemia .
	manualset3
119193	2	403949	13	NULL	NULL	0	NULL	high CRP levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Obese children tended to have high CRP levels , BP elevation , and slight dyslipidemia .
	manualset3
119194	3	403949	13	NULL	NULL	0	NULL	BP elevation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Obese children tended to have high CRP levels , BP elevation , and slight dyslipidemia .
	manualset3
119195	4	403949	13	NULL	NULL	0	NULL	slight dyslipidemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Obese children tended to have high CRP levels , BP elevation , and slight dyslipidemia .
	manualset3
119196	1	403950	13	NULL	NULL	0	NULL	Obesity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity , clinical coronary heart disease , and an abnormal electrocardiogram at the time of diagnosis of diabetes mellitus were not associated with a significantly increased frequency of TIA or stroke .
	manualset3
119197	2	403950	13	NULL	NULL	0	NULL	clinical coronary heart disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity , clinical coronary heart disease , and an abnormal electrocardiogram at the time of diagnosis of diabetes mellitus were not associated with a significantly increased frequency of TIA or stroke .
	manualset3
119198	3	403950	13	NULL	NULL	0	NULL	abnormal electrocardiogram 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity , clinical coronary heart disease , and an abnormal electrocardiogram at the time of diagnosis of diabetes mellitus were not associated with a significantly increased frequency of TIA or stroke .
	manualset3
119199	4	403950	13	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity , clinical coronary heart disease , and an abnormal electrocardiogram at the time of diagnosis of diabetes mellitus were not associated with a significantly increased frequency of TIA or stroke .
	manualset3
119200	5	403950	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity , clinical coronary heart disease , and an abnormal electrocardiogram at the time of diagnosis of diabetes mellitus were not associated with a significantly increased frequency of TIA or stroke .
	manualset3
119201	6	403950	13	NULL	NULL	0	NULL	diabetes mellitus 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity , clinical coronary heart disease , and an abnormal electrocardiogram at the time of diagnosis of diabetes mellitus were not associated with a significantly increased frequency of TIA or stroke .
	manualset3
119202	7	403950	13	NULL	NULL	0	NULL	frequency of TIA 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity , clinical coronary heart disease , and an abnormal electrocardiogram at the time of diagnosis of diabetes mellitus were not associated with a significantly increased frequency of TIA or stroke .
	manualset3
119203	8	403950	13	NULL	NULL	0	NULL	stroke	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity , clinical coronary heart disease , and an abnormal electrocardiogram at the time of diagnosis of diabetes mellitus were not associated with a significantly increased frequency of TIA or stroke .
	manualset3
119412	1	403951	13	NULL	NULL	0	NULL	Obesity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity , especially waist-hip ratio , was a strong correlate of both total and free testosterone , but not of estradiol .
	manualset3
119413	2	403951	13	NULL	NULL	0	NULL	waist-hip ratio	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity , especially waist-hip ratio , was a strong correlate of both total and free testosterone , but not of estradiol .
	manualset3
119414	3	403951	13	NULL	NULL	0	NULL	total testosterone	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity , especially waist-hip ratio , was a strong correlate of both total and free testosterone , but not of estradiol .
	manualset3
119415	4	403951	13	NULL	NULL	0	NULL	free testosterone	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity , especially waist-hip ratio , was a strong correlate of both total and free testosterone , but not of estradiol .
	manualset3
119416	5	403951	13	NULL	NULL	0	NULL	estradiol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity , especially waist-hip ratio , was a strong correlate of both total and free testosterone , but not of estradiol .
	manualset3
119417	1	403952	13	NULL	NULL	0	NULL	Obesity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity is associated with increased cardiovascular disease .
	manualset3
119418	2	403952	13	NULL	NULL	0	NULL	cardiovascular disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity is associated with increased cardiovascular disease .
	manualset3
119419	1	403953	13	NULL	NULL	0	NULL	Obesity measures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity measures , blood pressure , fasting plasma glucose ( FPG ) , and 30 min of brisk walking were recorded for each participant .
	manualset3
119420	2	403953	13	NULL	NULL	0	NULL	blood pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity measures , blood pressure , fasting plasma glucose ( FPG ) , and 30 min of brisk walking were recorded for each participant .
	manualset3
119421	3	403953	13	NULL	NULL	0	NULL	fasting plasma glucose ( FPG ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity measures , blood pressure , fasting plasma glucose ( FPG ) , and 30 min of brisk walking were recorded for each participant .
	manualset3
119422	4	403953	13	NULL	NULL	0	NULL	30 min	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity measures , blood pressure , fasting plasma glucose ( FPG ) , and 30 min of brisk walking were recorded for each participant .
	manualset3
119423	5	403953	13	NULL	NULL	0	NULL	brisk walking	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity measures , blood pressure , fasting plasma glucose ( FPG ) , and 30 min of brisk walking were recorded for each participant .
	manualset3
119424	6	403953	13	NULL	NULL	0	NULL	participant	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Obesity measures , blood pressure , fasting plasma glucose ( FPG ) , and 30 min of brisk walking were recorded for each participant .
	manualset3
119719	1	403954	13	NULL	NULL	0	NULL	impact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective : To determine the impact of pharmacist counseling on patients ' knowledge of emergency contraception ( EC ) .
	manualset3
119720	2	403954	13	NULL	NULL	0	NULL	Objective	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective : To determine the impact of pharmacist counseling on patients ' knowledge of emergency contraception ( EC ) .
	manualset3
119721	3	403954	13	NULL	NULL	0	NULL	pharmacist counseling	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective : To determine the impact of pharmacist counseling on patients ' knowledge of emergency contraception ( EC ) .
	manualset3
119722	4	403954	13	NULL	NULL	0	NULL	patients '	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective : To determine the impact of pharmacist counseling on patients ' knowledge of emergency contraception ( EC ) .
	manualset3
119723	5	403954	13	NULL	NULL	0	NULL	knowledge 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective : To determine the impact of pharmacist counseling on patients ' knowledge of emergency contraception ( EC ) .
	manualset3
119724	6	403954	13	NULL	NULL	0	NULL	emergency contraception ( EC ) 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective : To determine the impact of pharmacist counseling on patients ' knowledge of emergency contraception ( EC ) .
	manualset3
119725	1	403955	13	NULL	NULL	0	NULL	Objective	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective : To examine in mice the acute effects of epigallocatechin gallate ( EGCG ) , a green tea bioactive polyphenol on substrate metabolism with focus on the fate of dietary lipids .
	manualset3
119726	2	403955	13	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective : To examine in mice the acute effects of epigallocatechin gallate ( EGCG ) , a green tea bioactive polyphenol on substrate metabolism with focus on the fate of dietary lipids .
	manualset3
119727	3	403955	13	NULL	NULL	0	NULL	acute effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective : To examine in mice the acute effects of epigallocatechin gallate ( EGCG ) , a green tea bioactive polyphenol on substrate metabolism with focus on the fate of dietary lipids .
	manualset3
119728	4	403955	13	NULL	NULL	0	NULL	epigallocatechin gallate ( EGCG )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective : To examine in mice the acute effects of epigallocatechin gallate ( EGCG ) , a green tea bioactive polyphenol on substrate metabolism with focus on the fate of dietary lipids .
	manualset3
119729	5	403955	13	NULL	NULL	0	NULL	green tea bioactive polyphenol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective : To examine in mice the acute effects of epigallocatechin gallate ( EGCG ) , a green tea bioactive polyphenol on substrate metabolism with focus on the fate of dietary lipids .
	manualset3
119730	6	403955	13	NULL	NULL	0	NULL	substrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective : To examine in mice the acute effects of epigallocatechin gallate ( EGCG ) , a green tea bioactive polyphenol on substrate metabolism with focus on the fate of dietary lipids .
	manualset3
119731	7	403955	13	NULL	NULL	0	NULL	metabolism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective : To examine in mice the acute effects of epigallocatechin gallate ( EGCG ) , a green tea bioactive polyphenol on substrate metabolism with focus on the fate of dietary lipids .
	manualset3
119732	8	403955	13	NULL	NULL	0	NULL	focus	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective : To examine in mice the acute effects of epigallocatechin gallate ( EGCG ) , a green tea bioactive polyphenol on substrate metabolism with focus on the fate of dietary lipids .
	manualset3
119733	9	403955	13	NULL	NULL	0	NULL	fate 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective : To examine in mice the acute effects of epigallocatechin gallate ( EGCG ) , a green tea bioactive polyphenol on substrate metabolism with focus on the fate of dietary lipids .
	manualset3
119734	10	403955	13	NULL	NULL	0	NULL	dietary lipids	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective : To examine in mice the acute effects of epigallocatechin gallate ( EGCG ) , a green tea bioactive polyphenol on substrate metabolism with focus on the fate of dietary lipids .
	manualset3
119735	1	403956	13	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A correlation between early levels of viremia and subsequent allograft injury suggests that initiation of antiviral therapy early in the posttransplant course might be desirable .
	manualset3
119736	2	403956	13	NULL	NULL	0	NULL	early levels of viremia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A correlation between early levels of viremia and subsequent allograft injury suggests that initiation of antiviral therapy early in the posttransplant course might be desirable .
	manualset3
119737	3	403956	13	NULL	NULL	0	NULL	allograft injury 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A correlation between early levels of viremia and subsequent allograft injury suggests that initiation of antiviral therapy early in the posttransplant course might be desirable .
	manualset3
119738	4	403956	13	NULL	NULL	0	NULL	initiation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A correlation between early levels of viremia and subsequent allograft injury suggests that initiation of antiviral therapy early in the posttransplant course might be desirable .
	manualset3
119739	5	403956	13	NULL	NULL	0	NULL	antiviral therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A correlation between early levels of viremia and subsequent allograft injury suggests that initiation of antiviral therapy early in the posttransplant course might be desirable .
	manualset3
119740	6	403956	13	NULL	NULL	0	NULL	posttransplant course	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A correlation between early levels of viremia and subsequent allograft injury suggests that initiation of antiviral therapy early in the posttransplant course might be desirable .
	manualset3
119741	1	403957	13	NULL	NULL	0	NULL	Objective	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective : We compared biological responses of cyanoacrylate anionic nanoparticles with cationic nanoparticles in cultured murine macrophages for assessing cytotoxicity and inflammatory responses .
	manualset3
119742	2	403957	13	NULL	NULL	0	NULL	biological responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective : We compared biological responses of cyanoacrylate anionic nanoparticles with cationic nanoparticles in cultured murine macrophages for assessing cytotoxicity and inflammatory responses .
	manualset3
119743	3	403957	13	NULL	NULL	0	NULL	cyanoacrylate anionic nanoparticles	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective : We compared biological responses of cyanoacrylate anionic nanoparticles with cationic nanoparticles in cultured murine macrophages for assessing cytotoxicity and inflammatory responses .
	manualset3
119744	4	403957	13	NULL	NULL	0	NULL	cationic nanoparticles	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective : We compared biological responses of cyanoacrylate anionic nanoparticles with cationic nanoparticles in cultured murine macrophages for assessing cytotoxicity and inflammatory responses .
	manualset3
119745	5	403957	13	NULL	NULL	0	NULL	murine macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective : We compared biological responses of cyanoacrylate anionic nanoparticles with cationic nanoparticles in cultured murine macrophages for assessing cytotoxicity and inflammatory responses .
	manualset3
119746	6	403957	13	NULL	NULL	0	NULL	cytotoxicity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective : We compared biological responses of cyanoacrylate anionic nanoparticles with cationic nanoparticles in cultured murine macrophages for assessing cytotoxicity and inflammatory responses .
	manualset3
119747	7	403957	13	NULL	NULL	0	NULL	inflammatory responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective : We compared biological responses of cyanoacrylate anionic nanoparticles with cationic nanoparticles in cultured murine macrophages for assessing cytotoxicity and inflammatory responses .
	manualset3
119748	1	403958	13	NULL	NULL	0	NULL	Objective analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective analysis versus subjective assessment of vowels pronounced by native , non-native , and deaf male speakers of Dutch .
	manualset3
119749	2	403958	13	NULL	NULL	0	NULL	subjective assessment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective analysis versus subjective assessment of vowels pronounced by native , non-native , and deaf male speakers of Dutch .
	manualset3
119777	3	403958	13	NULL	NULL	0	NULL	vowels	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective analysis versus subjective assessment of vowels pronounced by native , non-native , and deaf male speakers of Dutch .
	manualset3
119778	4	403958	13	NULL	NULL	0	NULL	native speakers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective analysis versus subjective assessment of vowels pronounced by native , non-native , and deaf male speakers of Dutch .
	manualset3
119779	5	403958	13	NULL	NULL	0	NULL	non-native speakers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective analysis versus subjective assessment of vowels pronounced by native , non-native , and deaf male speakers of Dutch .
	manualset3
119780	6	403958	13	NULL	NULL	0	NULL	deaf male speakers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective analysis versus subjective assessment of vowels pronounced by native , non-native , and deaf male speakers of Dutch .
	manualset3
119781	7	403958	13	NULL	NULL	0	NULL	Dutch 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective analysis versus subjective assessment of vowels pronounced by native , non-native , and deaf male speakers of Dutch .
	manualset3
119782	1	403959	13	NULL	NULL	0	NULL	Objective results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective results are reviewed individually for each test , with the overall combined result of static and moving two-point discrimination being excellent ( Highet S4 ) in 81 % for class I , 41 % for class II , and 31 % for class III , all different at a statistically significant level .
	manualset3
119783	2	403959	13	NULL	NULL	0	NULL	test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective results are reviewed individually for each test , with the overall combined result of static and moving two-point discrimination being excellent ( Highet S4 ) in 81 % for class I , 41 % for class II , and 31 % for class III , all different at a statistically significant level .
	manualset3
119784	3	403959	13	NULL	NULL	0	NULL	result 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective results are reviewed individually for each test , with the overall combined result of static and moving two-point discrimination being excellent ( Highet S4 ) in 81 % for class I , 41 % for class II , and 31 % for class III , all different at a statistically significant level .
	manualset3
119785	4	403959	13	NULL	NULL	0	NULL	two-point discrimination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective results are reviewed individually for each test , with the overall combined result of static and moving two-point discrimination being excellent ( Highet S4 ) in 81 % for class I , 41 % for class II , and 31 % for class III , all different at a statistically significant level .
	manualset3
119786	5	403959	13	NULL	NULL	0	NULL	Highet S4 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective results are reviewed individually for each test , with the overall combined result of static and moving two-point discrimination being excellent ( Highet S4 ) in 81 % for class I , 41 % for class II , and 31 % for class III , all different at a statistically significant level .
	manualset3
119787	6	403959	13	NULL	NULL	0	NULL	81 % for class I 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective results are reviewed individually for each test , with the overall combined result of static and moving two-point discrimination being excellent ( Highet S4 ) in 81 % for class I , 41 % for class II , and 31 % for class III , all different at a statistically significant level .
	manualset3
119788	7	403959	13	NULL	NULL	0	NULL	41 % for class II	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective results are reviewed individually for each test , with the overall combined result of static and moving two-point discrimination being excellent ( Highet S4 ) in 81 % for class I , 41 % for class II , and 31 % for class III , all different at a statistically significant level .
	manualset3
119789	8	403959	13	NULL	NULL	0	NULL	31 % for class III 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective results are reviewed individually for each test , with the overall combined result of static and moving two-point discrimination being excellent ( Highet S4 ) in 81 % for class I , 41 % for class II , and 31 % for class III , all different at a statistically significant level .
	manualset3
119790	9	403959	13	NULL	NULL	0	NULL	level 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective results are reviewed individually for each test , with the overall combined result of static and moving two-point discrimination being excellent ( Highet S4 ) in 81 % for class I , 41 % for class II , and 31 % for class III , all different at a statistically significant level .
	manualset3
119791	1	403960	13	NULL	NULL	0	NULL	Objectives	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Objectives : The purpose of this study was to determine the sensitivity of breast-specific gamma imaging ( BSGI ) in the detection of invasive breast cancers and to characterise the sensitivity of BSGI based on tumor size and pathological grade .
	manualset3
119792	2	403960	13	NULL	NULL	0	NULL	purpose 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Objectives : The purpose of this study was to determine the sensitivity of breast-specific gamma imaging ( BSGI ) in the detection of invasive breast cancers and to characterise the sensitivity of BSGI based on tumor size and pathological grade .
	manualset3
119793	3	403960	13	NULL	NULL	NULL	NULL	study 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Objectives : The purpose of this study was to determine the sensitivity of breast-specific gamma imaging ( BSGI ) in the detection of invasive breast cancers and to characterise the sensitivity of BSGI based on tumor size and pathological grade .
	manualset3
119794	4	403960	13	NULL	NULL	0	NULL	sensitivity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Objectives : The purpose of this study was to determine the sensitivity of breast-specific gamma imaging ( BSGI ) in the detection of invasive breast cancers and to characterise the sensitivity of BSGI based on tumor size and pathological grade .
	manualset3
119795	5	403960	13	NULL	NULL	0	NULL	breast-specific gamma imaging ( BSGI ) 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Objectives : The purpose of this study was to determine the sensitivity of breast-specific gamma imaging ( BSGI ) in the detection of invasive breast cancers and to characterise the sensitivity of BSGI based on tumor size and pathological grade .
	manualset3
119796	6	403960	13	NULL	NULL	0	NULL	detection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Objectives : The purpose of this study was to determine the sensitivity of breast-specific gamma imaging ( BSGI ) in the detection of invasive breast cancers and to characterise the sensitivity of BSGI based on tumor size and pathological grade .
	manualset3
119797	7	403960	13	NULL	NULL	0	NULL	invasive breast cancers	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Objectives : The purpose of this study was to determine the sensitivity of breast-specific gamma imaging ( BSGI ) in the detection of invasive breast cancers and to characterise the sensitivity of BSGI based on tumor size and pathological grade .
	manualset3
119798	8	403960	13	NULL	NULL	0	NULL	sensitivity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Objectives : The purpose of this study was to determine the sensitivity of breast-specific gamma imaging ( BSGI ) in the detection of invasive breast cancers and to characterise the sensitivity of BSGI based on tumor size and pathological grade .
	manualset3
119799	9	403960	13	NULL	NULL	0	NULL	BSGI	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Objectives : The purpose of this study was to determine the sensitivity of breast-specific gamma imaging ( BSGI ) in the detection of invasive breast cancers and to characterise the sensitivity of BSGI based on tumor size and pathological grade .
	manualset3
119800	10	403960	13	NULL	NULL	0	NULL	tumor size	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Objectives : The purpose of this study was to determine the sensitivity of breast-specific gamma imaging ( BSGI ) in the detection of invasive breast cancers and to characterise the sensitivity of BSGI based on tumor size and pathological grade .
	manualset3
119801	11	403960	13	NULL	NULL	0	NULL	pathological grade	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Objectives : The purpose of this study was to determine the sensitivity of breast-specific gamma imaging ( BSGI ) in the detection of invasive breast cancers and to characterise the sensitivity of BSGI based on tumor size and pathological grade .
	manualset3
119802	1	403961	13	NULL	NULL	0	NULL	Oblique section reconstruction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Oblique section reconstruction provides an alternative to tomography for 3-D imaging of crystalline objects with large unit cells .
	manualset3
119803	2	403961	13	NULL	NULL	0	NULL	tomography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Oblique section reconstruction provides an alternative to tomography for 3-D imaging of crystalline objects with large unit cells .
	manualset3
119804	3	403961	13	NULL	NULL	0	NULL	3-D imaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Oblique section reconstruction provides an alternative to tomography for 3-D imaging of crystalline objects with large unit cells .
	manualset3
119805	4	403961	13	NULL	NULL	0	NULL	crystalline objects 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Oblique section reconstruction provides an alternative to tomography for 3-D imaging of crystalline objects with large unit cells .
	manualset3
119806	5	403961	13	NULL	NULL	0	NULL	large unit cells 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Oblique section reconstruction provides an alternative to tomography for 3-D imaging of crystalline objects with large unit cells .
	manualset3
119807	1	403962	13	NULL	NULL	0	NULL	Observation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Observation of a propagation mode of a fiber fuse with a long-period damage track in hole-assisted fiber .
	manualset3
119808	2	403962	13	NULL	NULL	0	NULL	propagation mode	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Observation of a propagation mode of a fiber fuse with a long-period damage track in hole-assisted fiber .
	manualset3
119809	3	403962	13	NULL	NULL	0	NULL	fiber fuse 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Observation of a propagation mode of a fiber fuse with a long-period damage track in hole-assisted fiber .
	manualset3
119810	4	403962	13	NULL	NULL	0	NULL	long-period damage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Observation of a propagation mode of a fiber fuse with a long-period damage track in hole-assisted fiber .
	manualset3
119811	5	403962	13	NULL	NULL	0	NULL	track 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Observation of a propagation mode of a fiber fuse with a long-period damage track in hole-assisted fiber .
	manualset3
119812	6	403962	13	NULL	NULL	0	NULL	hole-assisted fiber	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Observation of a propagation mode of a fiber fuse with a long-period damage track in hole-assisted fiber .
	manualset3
119813	1	403963	13	NULL	NULL	0	NULL	practice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A cost-effective , reusable practice eye model for epiretinal membrane peeling that uses easily obtained , commercially available materials was developed .
	manualset3
119814	2	403963	13	NULL	NULL	0	NULL	eye model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A cost-effective , reusable practice eye model for epiretinal membrane peeling that uses easily obtained , commercially available materials was developed .
	manualset3
119815	3	403963	13	NULL	NULL	0	NULL	epiretinal membrane peeling	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A cost-effective , reusable practice eye model for epiretinal membrane peeling that uses easily obtained , commercially available materials was developed .
	manualset3
119816	4	403963	13	NULL	NULL	0	NULL	materials 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A cost-effective , reusable practice eye model for epiretinal membrane peeling that uses easily obtained , commercially available materials was developed .
	manualset3
119817	1	403964	13	NULL	NULL	0	NULL	Observation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Observation on 105 cases of duodenal bulbar ulcer treated by combined therapy of catgut embedding and Chinese drugs .
	manualset3
119818	2	403964	13	NULL	NULL	0	NULL	105 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Observation on 105 cases of duodenal bulbar ulcer treated by combined therapy of catgut embedding and Chinese drugs .
	manualset3
119819	3	403964	13	NULL	NULL	0	NULL	duodenal bulbar ulcer	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Observation on 105 cases of duodenal bulbar ulcer treated by combined therapy of catgut embedding and Chinese drugs .
	manualset3
119820	4	403964	13	NULL	NULL	0	NULL	combined therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Observation on 105 cases of duodenal bulbar ulcer treated by combined therapy of catgut embedding and Chinese drugs .
	manualset3
119821	5	403964	13	NULL	NULL	0	NULL	catgut embedding	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Observation on 105 cases of duodenal bulbar ulcer treated by combined therapy of catgut embedding and Chinese drugs .
	manualset3
119822	6	403964	13	NULL	NULL	0	NULL	Chinese drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Observation on 105 cases of duodenal bulbar ulcer treated by combined therapy of catgut embedding and Chinese drugs .
	manualset3
119823	1	403965	13	NULL	NULL	0	NULL	Observations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Observations on the pathogenic effects of Trichuris ovis in sheep under drought conditions .
	manualset3
119824	2	403965	13	NULL	NULL	0	NULL	pathogenic effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Observations on the pathogenic effects of Trichuris ovis in sheep under drought conditions .
	manualset3
119825	3	403965	13	NULL	NULL	0	NULL	Trichuris ovis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Observations on the pathogenic effects of Trichuris ovis in sheep under drought conditions .
	manualset3
119826	4	403965	13	NULL	NULL	0	NULL	sheep 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Observations on the pathogenic effects of Trichuris ovis in sheep under drought conditions .
	manualset3
119827	5	403965	13	NULL	NULL	0	NULL	drought conditions	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Observations on the pathogenic effects of Trichuris ovis in sheep under drought conditions .
	manualset3
119828	1	403966	13	NULL	NULL	0	NULL	Observations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Observations suggest that tumor progression may in part require autocrine stimulation of the epithelia .
	manualset3
119829	2	403966	13	NULL	NULL	0	NULL	tumor progression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Observations suggest that tumor progression may in part require autocrine stimulation of the epithelia .
	manualset3
119830	3	403966	13	NULL	NULL	0	NULL	autocrine stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Observations suggest that tumor progression may in part require autocrine stimulation of the epithelia .
	manualset3
119831	4	403966	13	NULL	NULL	0	NULL	epithelia	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Observations suggest that tumor progression may in part require autocrine stimulation of the epithelia .
	manualset3
119832	1	403967	13	NULL	NULL	0	NULL	cost-minimization analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A cost-minimization analysis found that , on average , costs of the DUI court exceeded traditional court expenditures for second-time offenders but produced cost savings for third-time offenders .
	manualset3
119833	2	403967	13	NULL	NULL	0	NULL	costs 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A cost-minimization analysis found that , on average , costs of the DUI court exceeded traditional court expenditures for second-time offenders but produced cost savings for third-time offenders .
	manualset3
119834	3	403967	13	NULL	NULL	0	NULL	DUI court	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A cost-minimization analysis found that , on average , costs of the DUI court exceeded traditional court expenditures for second-time offenders but produced cost savings for third-time offenders .
	manualset3
119835	4	403967	13	NULL	NULL	0	NULL	traditional court expenditures	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A cost-minimization analysis found that , on average , costs of the DUI court exceeded traditional court expenditures for second-time offenders but produced cost savings for third-time offenders .
	manualset3
119836	5	403967	13	NULL	NULL	0	NULL	second-time offenders	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A cost-minimization analysis found that , on average , costs of the DUI court exceeded traditional court expenditures for second-time offenders but produced cost savings for third-time offenders .
	manualset3
119837	6	403967	13	NULL	NULL	0	NULL	cost savings	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A cost-minimization analysis found that , on average , costs of the DUI court exceeded traditional court expenditures for second-time offenders but produced cost savings for third-time offenders .
	manualset3
119838	7	403967	13	NULL	NULL	0	NULL	third-time offenders	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A cost-minimization analysis found that , on average , costs of the DUI court exceeded traditional court expenditures for second-time offenders but produced cost savings for third-time offenders .
	manualset3
119839	1	403968	13	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Observed differences among suits were statistically significant at p = 0.27 for the heat stress experiment , and extended over the range p = 0.003-0 .500 for the penetration experiment .
	manualset3
119840	2	403968	13	NULL	NULL	0	NULL	suits	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Observed differences among suits were statistically significant at p = 0.27 for the heat stress experiment , and extended over the range p = 0.003-0 .500 for the penetration experiment .
	manualset3
119841	3	403968	13	NULL	NULL	0	NULL	p = 0.27 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Observed differences among suits were statistically significant at p = 0.27 for the heat stress experiment , and extended over the range p = 0.003-0 .500 for the penetration experiment .
	manualset3
119842	4	403968	13	NULL	NULL	0	NULL	heat stress experiment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Observed differences among suits were statistically significant at p = 0.27 for the heat stress experiment , and extended over the range p = 0.003-0 .500 for the penetration experiment .
	manualset3
119843	5	403968	13	NULL	NULL	0	NULL	range p = 0.003-0 .500	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Observed differences among suits were statistically significant at p = 0.27 for the heat stress experiment , and extended over the range p = 0.003-0 .500 for the penetration experiment .
	manualset3
119844	6	403968	13	NULL	NULL	0	NULL	penetration experiment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Observed differences among suits were statistically significant at p = 0.27 for the heat stress experiment , and extended over the range p = 0.003-0 .500 for the penetration experiment .
	manualset3
119845	1	403969	13	NULL	NULL	0	NULL	Obstacles 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Obstacles , such as a lack of human resources , productivity goals and lack of training in mental health of FHS professionals were mentioned .
	manualset3
119846	2	403969	13	NULL	NULL	0	NULL	lack	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Obstacles , such as a lack of human resources , productivity goals and lack of training in mental health of FHS professionals were mentioned .
	manualset3
119847	3	403969	13	NULL	NULL	0	NULL	human resources	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Obstacles , such as a lack of human resources , productivity goals and lack of training in mental health of FHS professionals were mentioned .
	manualset3
119848	4	403969	13	NULL	NULL	0	NULL	productivity goals 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Obstacles , such as a lack of human resources , productivity goals and lack of training in mental health of FHS professionals were mentioned .
	manualset3
119849	5	403969	13	NULL	NULL	0	NULL	lack of training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Obstacles , such as a lack of human resources , productivity goals and lack of training in mental health of FHS professionals were mentioned .
	manualset3
119850	6	403969	13	NULL	NULL	0	NULL	mental health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Obstacles , such as a lack of human resources , productivity goals and lack of training in mental health of FHS professionals were mentioned .
	manualset3
119851	7	403969	13	NULL	NULL	0	NULL	FHS professionals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Obstacles , such as a lack of human resources , productivity goals and lack of training in mental health of FHS professionals were mentioned .
	manualset3
119852	1	403970	13	NULL	NULL	0	NULL	Obstacles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Obstacles in implementation of higher unit dosage of psychotropics drugs .
	manualset3
119853	2	403970	13	NULL	NULL	0	NULL	implementation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Obstacles in implementation of higher unit dosage of psychotropics drugs .
	manualset3
119854	3	403970	13	NULL	NULL	0	NULL	higher unit dosage 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Obstacles in implementation of higher unit dosage of psychotropics drugs .
	manualset3
119855	4	403970	13	NULL	NULL	0	NULL	psychotropics drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Obstacles in implementation of higher unit dosage of psychotropics drugs .
	manualset3
119856	1	403971	13	NULL	NULL	0	NULL	Obstetric US imaging 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Obstetric US imaging : the past 40 years .
	manualset3
119857	2	403971	13	NULL	NULL	0	NULL	past 40 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Obstetric US imaging : the past 40 years .
	manualset3
119858	1	403972	13	NULL	NULL	0	NULL	Obstructive sleep apnoea syndrome ( OSA ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Obstructive sleep apnoea syndrome ( OSA ) is associated with increased cardiovascular morbidity and mortality .
	manualset3
119859	2	403972	13	NULL	NULL	0	NULL	cardiovascular morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Obstructive sleep apnoea syndrome ( OSA ) is associated with increased cardiovascular morbidity and mortality .
	manualset3
119860	3	403972	13	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Obstructive sleep apnoea syndrome ( OSA ) is associated with increased cardiovascular morbidity and mortality .
	manualset3
119861	1	403973	13	NULL	NULL	0	NULL	menu	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Obviously , this menu is not comprehensive and many other topics could have been selected for emphasis .
	manualset3
119862	2	403973	13	NULL	NULL	0	NULL	topics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Obviously , this menu is not comprehensive and many other topics could have been selected for emphasis .
	manualset3
119863	3	403973	13	NULL	NULL	0	NULL	emphasis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Obviously , this menu is not comprehensive and many other topics could have been selected for emphasis .
	manualset3
119864	1	403974	13	NULL	NULL	0	NULL	symptomatic patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Obviously the symptomatic patients have to undergo hysteroscopy as soon as possible as a higher incidence of HRH and endometrial carcinoma has been detected in this group of patients .
	manualset3
119865	2	403974	13	NULL	NULL	0	NULL	hysteroscopy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Obviously the symptomatic patients have to undergo hysteroscopy as soon as possible as a higher incidence of HRH and endometrial carcinoma has been detected in this group of patients .
	manualset3
119866	3	403974	13	NULL	NULL	0	NULL	higher incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Obviously the symptomatic patients have to undergo hysteroscopy as soon as possible as a higher incidence of HRH and endometrial carcinoma has been detected in this group of patients .
	manualset3
119867	4	403974	13	NULL	NULL	0	NULL	HRH	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Obviously the symptomatic patients have to undergo hysteroscopy as soon as possible as a higher incidence of HRH and endometrial carcinoma has been detected in this group of patients .
	manualset3
119868	5	403974	13	NULL	NULL	0	NULL	endometrial carcinoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Obviously the symptomatic patients have to undergo hysteroscopy as soon as possible as a higher incidence of HRH and endometrial carcinoma has been detected in this group of patients .
	manualset3
119869	6	403974	13	NULL	NULL	0	NULL	group of patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Obviously the symptomatic patients have to undergo hysteroscopy as soon as possible as a higher incidence of HRH and endometrial carcinoma has been detected in this group of patients .
	manualset3
119870	1	403975	13	NULL	NULL	0	NULL	CGRP-containing nerve fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Occasional CGRP-containing nerve fibers were also noted adjacent to submucosal gland acini , near the epithelial basement membrane , and between epithelial cells .
	manualset3
119871	2	403975	13	NULL	NULL	0	NULL	submucosal gland acini 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Occasional CGRP-containing nerve fibers were also noted adjacent to submucosal gland acini , near the epithelial basement membrane , and between epithelial cells .
	manualset3
119872	3	403975	13	NULL	NULL	0	NULL	epithelial basement membrane	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Occasional CGRP-containing nerve fibers were also noted adjacent to submucosal gland acini , near the epithelial basement membrane , and between epithelial cells .
	manualset3
119873	4	403975	13	NULL	NULL	0	NULL	epithelial cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Occasional CGRP-containing nerve fibers were also noted adjacent to submucosal gland acini , near the epithelial basement membrane , and between epithelial cells .
	manualset3
119874	1	403976	13	NULL	NULL	0	NULL	parent 's rating 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Occasionally , however , a parent 's rating may differ from a teacher 's sufficiently to lead to a different classification .
	manualset3
119875	2	403976	13	NULL	NULL	0	NULL	teacher 's 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Occasionally , however , a parent 's rating may differ from a teacher 's sufficiently to lead to a different classification .
	manualset3
119876	3	403976	13	NULL	NULL	0	NULL	classification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Occasionally , however , a parent 's rating may differ from a teacher 's sufficiently to lead to a different classification .
	manualset3
119877	1	403977	13	NULL	NULL	0	NULL	cost comparison	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A cost comparison of liver transplantation with FK 506 or CyA as the primary immunosuppressive agent .
	manualset3
119878	2	403977	13	NULL	NULL	0	NULL	liver transplantation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A cost comparison of liver transplantation with FK 506 or CyA as the primary immunosuppressive agent .
	manualset3
119879	3	403977	13	NULL	NULL	0	NULL	FK 506	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A cost comparison of liver transplantation with FK 506 or CyA as the primary immunosuppressive agent .
	manualset3
119880	4	403977	13	NULL	NULL	0	NULL	CyA 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A cost comparison of liver transplantation with FK 506 or CyA as the primary immunosuppressive agent .
	manualset3
119881	5	403977	13	NULL	NULL	0	NULL	primary immunosuppressive agent	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A cost comparison of liver transplantation with FK 506 or CyA as the primary immunosuppressive agent .
	manualset3
119882	1	403978	13	NULL	NULL	0	NULL	Occipital peripheral nerve 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Occipital peripheral nerve stimulation in the management of chronic intractable occipital neuralgia in a patient with neurofibromatosis type 1 : a case report .
	manualset3
119883	2	403978	13	NULL	NULL	0	NULL	stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Occipital peripheral nerve stimulation in the management of chronic intractable occipital neuralgia in a patient with neurofibromatosis type 1 : a case report .
	manualset3
119884	3	403978	13	NULL	NULL	0	NULL	management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Occipital peripheral nerve stimulation in the management of chronic intractable occipital neuralgia in a patient with neurofibromatosis type 1 : a case report .
	manualset3
119885	4	403978	13	NULL	NULL	0	NULL	chronic intractable occipital neuralgia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Occipital peripheral nerve stimulation in the management of chronic intractable occipital neuralgia in a patient with neurofibromatosis type 1 : a case report .
	manualset3
119886	5	403978	13	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Occipital peripheral nerve stimulation in the management of chronic intractable occipital neuralgia in a patient with neurofibromatosis type 1 : a case report .
	manualset3
119887	6	403978	13	NULL	NULL	0	NULL	neurofibromatosis type 1	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Occipital peripheral nerve stimulation in the management of chronic intractable occipital neuralgia in a patient with neurofibromatosis type 1 : a case report .
	manualset3
119888	7	403978	13	NULL	NULL	0	NULL	case report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Occipital peripheral nerve stimulation in the management of chronic intractable occipital neuralgia in a patient with neurofibromatosis type 1 : a case report .
	manualset3
119889	1	403979	13	NULL	NULL	0	NULL	Occipital condylar fractures 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Occipital condylar fractures : a review .
	manualset3
119890	2	403979	13	NULL	NULL	0	NULL	review 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Occipital condylar fractures : a review .
	manualset3
119891	1	403980	13	NULL	NULL	0	NULL	Occlusion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Occlusion with a vapour-impermeable wrap blocked restoration of the Ca2 + gradient after acute barrier disruption .
	manualset3
119892	2	403980	13	NULL	NULL	0	NULL	restoration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Occlusion with a vapour-impermeable wrap blocked restoration of the Ca2 + gradient after acute barrier disruption .
	manualset3
119893	3	403980	13	NULL	NULL	0	NULL	Ca2 + gradient	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Occlusion with a vapour-impermeable wrap blocked restoration of the Ca2 + gradient after acute barrier disruption .
	manualset3
119894	4	403980	13	NULL	NULL	0	NULL	acute barrier disruption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Occlusion with a vapour-impermeable wrap blocked restoration of the Ca2 + gradient after acute barrier disruption .
	manualset3
119895	1	403981	13	NULL	NULL	0	NULL	Occlusions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Occlusions of the superior mesenteric artery for periods of more than 60 min resulted in significant leakage of 125I-albumin ( i.v. ) into the lumen .
	manualset3
119896	2	403981	13	NULL	NULL	0	NULL	superior mesenteric artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Occlusions of the superior mesenteric artery for periods of more than 60 min resulted in significant leakage of 125I-albumin ( i.v. ) into the lumen .
	manualset3
119897	3	403981	13	NULL	NULL	0	NULL	periods	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Occlusions of the superior mesenteric artery for periods of more than 60 min resulted in significant leakage of 125I-albumin ( i.v. ) into the lumen .
	manualset3
119898	4	403981	13	NULL	NULL	0	NULL	60 min	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Occlusions of the superior mesenteric artery for periods of more than 60 min resulted in significant leakage of 125I-albumin ( i.v. ) into the lumen .
	manualset3
119899	5	403981	13	NULL	NULL	0	NULL	leakage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Occlusions of the superior mesenteric artery for periods of more than 60 min resulted in significant leakage of 125I-albumin ( i.v. ) into the lumen .
	manualset3
119900	6	403981	13	NULL	NULL	0	NULL	125I-albumin ( i.v. )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Occlusions of the superior mesenteric artery for periods of more than 60 min resulted in significant leakage of 125I-albumin ( i.v. ) into the lumen .
	manualset3
119901	7	403981	13	NULL	NULL	0	NULL	lumen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Occlusions of the superior mesenteric artery for periods of more than 60 min resulted in significant leakage of 125I-albumin ( i.v. ) into the lumen .
	manualset3
119902	1	403982	13	NULL	NULL	0	NULL	Occult distant metastases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Occult distant metastases of well-differentiated thyroid carcinoma .
	manualset3
119903	2	403982	13	NULL	NULL	0	NULL	thyroid carcinoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Occult distant metastases of well-differentiated thyroid carcinoma .
	manualset3
119904	1	403983	13	NULL	NULL	0	NULL	Occult gastrointestinal bleeding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Occult gastrointestinal bleeding as measured by the faecal 51Cr-labelled red-cell loss was compared in eight healthy volunteers while on therapeutic doses of soluble aspirin and a new slow-release formulation of aspirin ( Deskoval ) .
	manualset3
119905	2	403983	13	NULL	NULL	0	NULL	faecal 51Cr-labelled red-cell loss 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Occult gastrointestinal bleeding as measured by the faecal 51Cr-labelled red-cell loss was compared in eight healthy volunteers while on therapeutic doses of soluble aspirin and a new slow-release formulation of aspirin ( Deskoval ) .
	manualset3
119906	3	403983	13	NULL	NULL	0	NULL	eight healthy volunteers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Occult gastrointestinal bleeding as measured by the faecal 51Cr-labelled red-cell loss was compared in eight healthy volunteers while on therapeutic doses of soluble aspirin and a new slow-release formulation of aspirin ( Deskoval ) .
	manualset3
119907	4	403983	13	NULL	NULL	0	NULL	therapeutic doses 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Occult gastrointestinal bleeding as measured by the faecal 51Cr-labelled red-cell loss was compared in eight healthy volunteers while on therapeutic doses of soluble aspirin and a new slow-release formulation of aspirin ( Deskoval ) .
	manualset3
119908	5	403983	13	NULL	NULL	0	NULL	soluble aspirin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Occult gastrointestinal bleeding as measured by the faecal 51Cr-labelled red-cell loss was compared in eight healthy volunteers while on therapeutic doses of soluble aspirin and a new slow-release formulation of aspirin ( Deskoval ) .
	manualset3
119909	6	403983	13	NULL	NULL	0	NULL	slow-release formulation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Occult gastrointestinal bleeding as measured by the faecal 51Cr-labelled red-cell loss was compared in eight healthy volunteers while on therapeutic doses of soluble aspirin and a new slow-release formulation of aspirin ( Deskoval ) .
	manualset3
119910	7	403983	13	NULL	NULL	0	NULL	aspirin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Occult gastrointestinal bleeding as measured by the faecal 51Cr-labelled red-cell loss was compared in eight healthy volunteers while on therapeutic doses of soluble aspirin and a new slow-release formulation of aspirin ( Deskoval ) .
	manualset3
119911	8	403983	13	NULL	NULL	0	NULL	Deskoval	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Occult gastrointestinal bleeding as measured by the faecal 51Cr-labelled red-cell loss was compared in eight healthy volunteers while on therapeutic doses of soluble aspirin and a new slow-release formulation of aspirin ( Deskoval ) .
	manualset3
119912	1	403984	13	NULL	NULL	0	NULL	Occult papillary thyroid carcinoma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Occult papillary thyroid carcinoma in Hashimoto 's thyroiditis presenting as a metastatic bone tumor .
	manualset3
119913	2	403984	13	NULL	NULL	0	NULL	Hashimoto 's thyroiditis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Occult papillary thyroid carcinoma in Hashimoto 's thyroiditis presenting as a metastatic bone tumor .
	manualset3
119914	3	403984	13	NULL	NULL	0	NULL	metastatic bone tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Occult papillary thyroid carcinoma in Hashimoto 's thyroiditis presenting as a metastatic bone tumor .
	manualset3
119915	1	403985	13	NULL	NULL	0	NULL	Occupational exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Occupational exposure to asbestos is involved in 70-80 % of all malignant pleural mesothelioma .
	manualset3
119916	2	403985	13	NULL	NULL	0	NULL	asbestos	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Occupational exposure to asbestos is involved in 70-80 % of all malignant pleural mesothelioma .
	manualset3
119917	3	403985	13	NULL	NULL	0	NULL	70-80 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Occupational exposure to asbestos is involved in 70-80 % of all malignant pleural mesothelioma .
	manualset3
119918	4	403985	13	NULL	NULL	0	NULL	malignant pleural mesothelioma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Occupational exposure to asbestos is involved in 70-80 % of all malignant pleural mesothelioma .
	manualset3
119919	1	403986	13	NULL	NULL	0	NULL	crisis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A crisis in chronic pain care : an ethical analysis .
	manualset3
119920	2	403986	13	NULL	NULL	0	NULL	chronic pain care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A crisis in chronic pain care : an ethical analysis .
	manualset3
119921	3	403986	13	NULL	NULL	0	NULL	ethical analysis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A crisis in chronic pain care : an ethical analysis .
	manualset3
119922	1	403987	13	NULL	NULL	0	NULL	Occupational therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Occupational therapy role on the battlefield : an overview of combat and operational stress and upper extremity rehabilitation .
	manualset3
119923	2	403987	13	NULL	NULL	0	NULL	role 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Occupational therapy role on the battlefield : an overview of combat and operational stress and upper extremity rehabilitation .
	manualset3
119924	3	403987	13	NULL	NULL	0	NULL	battlefield	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Occupational therapy role on the battlefield : an overview of combat and operational stress and upper extremity rehabilitation .
	manualset3
119925	4	403987	13	NULL	NULL	0	NULL	overview	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Occupational therapy role on the battlefield : an overview of combat and operational stress and upper extremity rehabilitation .
	manualset3
119926	5	403987	13	NULL	NULL	0	NULL	combat	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Occupational therapy role on the battlefield : an overview of combat and operational stress and upper extremity rehabilitation .
	manualset3
119927	6	403987	13	NULL	NULL	0	NULL	operational stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Occupational therapy role on the battlefield : an overview of combat and operational stress and upper extremity rehabilitation .
	manualset3
119928	7	403987	13	NULL	NULL	0	NULL	upper extremity rehabilitation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Occupational therapy role on the battlefield : an overview of combat and operational stress and upper extremity rehabilitation .
	manualset3
119929	1	403988	13	NULL	NULL	0	NULL	Occupational asthma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Occupational asthma is recognized as the most common form of occupational lung disease .
	manualset3
119930	2	403988	13	NULL	NULL	0	NULL	common form 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Occupational asthma is recognized as the most common form of occupational lung disease .
	manualset3
119931	3	403988	13	NULL	NULL	0	NULL	occupational lung disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Occupational asthma is recognized as the most common form of occupational lung disease .
	manualset3
119932	1	403989	13	NULL	NULL	0	NULL	Occurrence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence and distribution of triclosan in the German Bight ( North Sea ) .
	manualset3
119933	2	403989	13	NULL	NULL	0	NULL	distribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence and distribution of triclosan in the German Bight ( North Sea ) .
	manualset3
119934	3	403989	13	NULL	NULL	0	NULL	triclosan	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence and distribution of triclosan in the German Bight ( North Sea ) .
	manualset3
119935	4	403989	13	NULL	NULL	0	NULL	German Bight 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence and distribution of triclosan in the German Bight ( North Sea ) .
	manualset3
119936	5	403989	13	NULL	NULL	0	NULL	North Sea	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence and distribution of triclosan in the German Bight ( North Sea ) .
	manualset3
119937	1	403990	13	NULL	NULL	0	NULL	Occurrence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence and fate of pharmaceuticals and alkylphenol ethoxylate metabolites in an effluent-dominated river and wetland .
	manualset3
119938	2	403990	13	NULL	NULL	0	NULL	fate	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence and fate of pharmaceuticals and alkylphenol ethoxylate metabolites in an effluent-dominated river and wetland .
	manualset3
119939	3	403990	13	NULL	NULL	0	NULL	pharmaceuticals 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence and fate of pharmaceuticals and alkylphenol ethoxylate metabolites in an effluent-dominated river and wetland .
	manualset3
119940	4	403990	13	NULL	NULL	0	NULL	alkylphenol ethoxylate metabolites 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence and fate of pharmaceuticals and alkylphenol ethoxylate metabolites in an effluent-dominated river and wetland .
	manualset3
119941	5	403990	13	NULL	NULL	0	NULL	effluent-dominated river	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence and fate of pharmaceuticals and alkylphenol ethoxylate metabolites in an effluent-dominated river and wetland .
	manualset3
119942	6	403990	13	NULL	NULL	0	NULL	wetland	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence and fate of pharmaceuticals and alkylphenol ethoxylate metabolites in an effluent-dominated river and wetland .
	manualset3
119943	1	403991	13	NULL	NULL	0	NULL	Occurrence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence of herbicides such as chlortoluron , isoproturon and terbuthylazine in surface water could be due to their broad agricultural application in regional dominant crops , such as barley , wheat and maize .
	manualset3
119944	2	403991	13	NULL	NULL	0	NULL	herbicides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence of herbicides such as chlortoluron , isoproturon and terbuthylazine in surface water could be due to their broad agricultural application in regional dominant crops , such as barley , wheat and maize .
	manualset3
119945	3	403991	13	NULL	NULL	0	NULL	chlortoluron 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence of herbicides such as chlortoluron , isoproturon and terbuthylazine in surface water could be due to their broad agricultural application in regional dominant crops , such as barley , wheat and maize .
	manualset3
119946	4	403991	13	NULL	NULL	0	NULL	isoproturon	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence of herbicides such as chlortoluron , isoproturon and terbuthylazine in surface water could be due to their broad agricultural application in regional dominant crops , such as barley , wheat and maize .
	manualset3
119947	5	403991	13	NULL	NULL	0	NULL	terbuthylazine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence of herbicides such as chlortoluron , isoproturon and terbuthylazine in surface water could be due to their broad agricultural application in regional dominant crops , such as barley , wheat and maize .
	manualset3
119948	6	403991	13	NULL	NULL	0	NULL	surface water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence of herbicides such as chlortoluron , isoproturon and terbuthylazine in surface water could be due to their broad agricultural application in regional dominant crops , such as barley , wheat and maize .
	manualset3
119949	7	403991	13	NULL	NULL	0	NULL	 agricultural application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence of herbicides such as chlortoluron , isoproturon and terbuthylazine in surface water could be due to their broad agricultural application in regional dominant crops , such as barley , wheat and maize .
	manualset3
119950	8	403991	13	NULL	NULL	0	NULL	regional dominant crops 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence of herbicides such as chlortoluron , isoproturon and terbuthylazine in surface water could be due to their broad agricultural application in regional dominant crops , such as barley , wheat and maize .
	manualset3
119951	9	403991	13	NULL	NULL	NULL	NULL	barley	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Occurrence of herbicides such as chlortoluron , isoproturon and terbuthylazine in surface water could be due to their broad agricultural application in regional dominant crops , such as barley , wheat and maize .
	manualset3
119952	10	403991	13	NULL	NULL	NULL	NULL	wheat	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Occurrence of herbicides such as chlortoluron , isoproturon and terbuthylazine in surface water could be due to their broad agricultural application in regional dominant crops , such as barley , wheat and maize .
	manualset3
119953	11	403991	13	NULL	NULL	NULL	NULL	maize	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Occurrence of herbicides such as chlortoluron , isoproturon and terbuthylazine in surface water could be due to their broad agricultural application in regional dominant crops , such as barley , wheat and maize .
	manualset3
119954	1	403992	13	NULL	NULL	0	NULL	Occurrence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence of thermotolerant Campylobacter spp .
	manualset3
119955	2	403992	13	NULL	NULL	0	NULL	 thermotolerant Campylobacter spp	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence of thermotolerant Campylobacter spp .
	manualset3
119956	1	403993	13	NULL	NULL	0	NULL	Occurrence sampling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence sampling was used in the main production area of a university residence hall foodservice to measure and analyze work functions involved in entre production and to determine time requirements for entre categories .
	manualset3
119957	2	403993	13	NULL	NULL	0	NULL	main production area	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence sampling was used in the main production area of a university residence hall foodservice to measure and analyze work functions involved in entre production and to determine time requirements for entre categories .
	manualset3
119958	3	403993	13	NULL	NULL	0	NULL	university residence hall 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence sampling was used in the main production area of a university residence hall foodservice to measure and analyze work functions involved in entre production and to determine time requirements for entre categories .
	manualset3
119959	4	403993	13	NULL	NULL	0	NULL	foodservice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence sampling was used in the main production area of a university residence hall foodservice to measure and analyze work functions involved in entre production and to determine time requirements for entre categories .
	manualset3
119960	5	403993	13	NULL	NULL	0	NULL	work functions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence sampling was used in the main production area of a university residence hall foodservice to measure and analyze work functions involved in entre production and to determine time requirements for entre categories .
	manualset3
119961	6	403993	13	NULL	NULL	0	NULL	entre production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence sampling was used in the main production area of a university residence hall foodservice to measure and analyze work functions involved in entre production and to determine time requirements for entre categories .
	manualset3
119962	7	403993	13	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence sampling was used in the main production area of a university residence hall foodservice to measure and analyze work functions involved in entre production and to determine time requirements for entre categories .
	manualset3
119963	8	403993	13	NULL	NULL	0	NULL	requirements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence sampling was used in the main production area of a university residence hall foodservice to measure and analyze work functions involved in entre production and to determine time requirements for entre categories .
	manualset3
119964	9	403993	13	NULL	NULL	0	NULL	entre categories	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence sampling was used in the main production area of a university residence hall foodservice to measure and analyze work functions involved in entre production and to determine time requirements for entre categories .
	manualset3
119965	1	403994	13	NULL	NULL	0	NULL	Oct-GnRH	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Oct-GnRH showed luteinising hormone-releasing activity in the anterior pituitary cells of the Japanese quail Coturnix coturnix .
	manualset3
119966	2	403994	13	NULL	NULL	0	NULL	luteinising hormone-releasing activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Oct-GnRH showed luteinising hormone-releasing activity in the anterior pituitary cells of the Japanese quail Coturnix coturnix .
	manualset3
119967	3	403994	13	NULL	NULL	0	NULL	anterior pituitary cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Oct-GnRH showed luteinising hormone-releasing activity in the anterior pituitary cells of the Japanese quail Coturnix coturnix .
	manualset3
119968	4	403994	13	NULL	NULL	0	NULL	Japanese quail Coturnix coturnix	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Oct-GnRH showed luteinising hormone-releasing activity in the anterior pituitary cells of the Japanese quail Coturnix coturnix .
	manualset3
119969	1	403995	13	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A critical role for Syk in endothelial cell proliferation and migration .
	manualset3
119970	2	403995	13	NULL	NULL	0	NULL	Syk	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A critical role for Syk in endothelial cell proliferation and migration .
	manualset3
119971	3	403995	13	NULL	NULL	0	NULL	endothelial cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A critical role for Syk in endothelial cell proliferation and migration .
	manualset3
119972	4	403995	13	NULL	NULL	0	NULL	migration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A critical role for Syk in endothelial cell proliferation and migration .
	manualset3
119973	1	403996	13	NULL	NULL	0	NULL	Octreotide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Octreotide for treatment of chylothorax after repair of congenital diaphragmatic hernia .
	manualset3
119974	2	403996	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Octreotide for treatment of chylothorax after repair of congenital diaphragmatic hernia .
	manualset3
119975	3	403996	13	NULL	NULL	0	NULL	chylothorax	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Octreotide for treatment of chylothorax after repair of congenital diaphragmatic hernia .
	manualset3
119976	4	403996	13	NULL	NULL	0	NULL	repair	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Octreotide for treatment of chylothorax after repair of congenital diaphragmatic hernia .
	manualset3
119977	5	403996	13	NULL	NULL	0	NULL	congenital diaphragmatic hernia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Octreotide for treatment of chylothorax after repair of congenital diaphragmatic hernia .
	manualset3
119978	1	403997	13	NULL	NULL	0	NULL	Octreotide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Octreotide treatment of idiopathic pulmonary fibrosis : a proof-of-concept study .
	manualset3
119979	2	403997	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Octreotide treatment of idiopathic pulmonary fibrosis : a proof-of-concept study .
	manualset3
119980	3	403997	13	NULL	NULL	0	NULL	idiopathic pulmonary fibrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Octreotide treatment of idiopathic pulmonary fibrosis : a proof-of-concept study .
	manualset3
119981	4	403997	13	NULL	NULL	0	NULL	proof-of-concept study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Octreotide treatment of idiopathic pulmonary fibrosis : a proof-of-concept study .
	manualset3
119982	1	403998	13	NULL	NULL	0	NULL	Ocular vascular disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Ocular vascular disease : in-office primary care diagnosis .
	manualset3
119983	2	403998	13	NULL	NULL	0	NULL	in-office primary care diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ocular vascular disease : in-office primary care diagnosis .
	manualset3
119984	1	403999	13	NULL	NULL	0	NULL	Odd-skipped 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Odd-skipped maintains prohemocyte potency and blocks blood cell development in Drosophila .
	manualset3
119985	2	403999	13	NULL	NULL	0	NULL	prohemocyte potency	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Odd-skipped maintains prohemocyte potency and blocks blood cell development in Drosophila .
	manualset3
119986	3	403999	13	NULL	NULL	0	NULL	blocks blood cell development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Odd-skipped maintains prohemocyte potency and blocks blood cell development in Drosophila .
	manualset3
119987	4	403999	13	NULL	NULL	0	NULL	Drosophila	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Odd-skipped maintains prohemocyte potency and blocks blood cell development in Drosophila .
	manualset3
119988	1	404000	13	NULL	NULL	0	NULL	Odds ratios ( OR )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Odds ratios ( OR ) and 95 % CI were calculated for green tea consumption measures and adjusted for age and other confounding factors .
	manualset3
119989	2	404000	13	NULL	NULL	0	NULL	95 % CI	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Odds ratios ( OR ) and 95 % CI were calculated for green tea consumption measures and adjusted for age and other confounding factors .
	manualset3
119990	3	404000	13	NULL	NULL	0	NULL	green tea 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Odds ratios ( OR ) and 95 % CI were calculated for green tea consumption measures and adjusted for age and other confounding factors .
	manualset3
119991	4	404000	13	NULL	NULL	NULL	NULL	consumption measures	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Odds ratios ( OR ) and 95 % CI were calculated for green tea consumption measures and adjusted for age and other confounding factors .
	manualset3
119992	5	404000	13	NULL	NULL	NULL	NULL	age 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Odds ratios ( OR ) and 95 % CI were calculated for green tea consumption measures and adjusted for age and other confounding factors .
	manualset3
119993	6	404000	13	NULL	NULL	0	NULL	confounding factors	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Odds ratios ( OR ) and 95 % CI were calculated for green tea consumption measures and adjusted for age and other confounding factors .
	manualset3
119994	1	404001	13	NULL	NULL	0	NULL	Odds ratios	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Odds ratios of HBsAg and HBV infection were 28.82 and 31.22 , respectively .
	manualset3
119995	2	404001	13	NULL	NULL	0	NULL	HBsAg	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Odds ratios of HBsAg and HBV infection were 28.82 and 31.22 , respectively .
	manualset3
119996	3	404001	13	NULL	NULL	0	NULL	HBV infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Odds ratios of HBsAg and HBV infection were 28.82 and 31.22 , respectively .
	manualset3
119997	4	404001	13	NULL	NULL	0	NULL	28.82 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Odds ratios of HBsAg and HBV infection were 28.82 and 31.22 , respectively .
	manualset3
119998	5	404001	13	NULL	NULL	0	NULL	31.22	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Odds ratios of HBsAg and HBV infection were 28.82 and 31.22 , respectively .
	manualset3
119999	1	404002	13	NULL	NULL	0	NULL	Odontoid hypoplasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Odontoid hypoplasia presenting as torticollis : a discussion of its significance .
	manualset3
120000	2	404002	13	NULL	NULL	0	NULL	torticollis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Odontoid hypoplasia presenting as torticollis : a discussion of its significance .
	manualset3
120001	3	404002	13	NULL	NULL	0	NULL	discussion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Odontoid hypoplasia presenting as torticollis : a discussion of its significance .
	manualset3
120002	4	404002	13	NULL	NULL	0	NULL	significance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Odontoid hypoplasia presenting as torticollis : a discussion of its significance .
	manualset3
120003	1	404003	13	NULL	NULL	0	NULL	Oesophagogastric cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Oesophagogastric cancer and surgical subspecialisation : how much work ?
	manualset3
120004	2	404003	13	NULL	NULL	0	NULL	surgical subspecialisation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Oesophagogastric cancer and surgical subspecialisation : how much work ?
	manualset3
120005	3	404003	13	NULL	NULL	0	NULL	work	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Oesophagogastric cancer and surgical subspecialisation : how much work ?
	manualset3
120009	1	404004	13	NULL	NULL	0	NULL	cross-sectional study 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A cross-sectional study involving 13 women with PCOS and 13 age - and body mass index-matched healthy controls was performed .
	manualset3
120010	2	404004	13	NULL	NULL	0	NULL	13 women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A cross-sectional study involving 13 women with PCOS and 13 age - and body mass index-matched healthy controls was performed .
	manualset3
120011	3	404004	13	NULL	NULL	0	NULL	PCOS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A cross-sectional study involving 13 women with PCOS and 13 age - and body mass index-matched healthy controls was performed .
	manualset3
120012	4	404004	13	NULL	NULL	0	NULL	13 age	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A cross-sectional study involving 13 women with PCOS and 13 age - and body mass index-matched healthy controls was performed .
	manualset3
120013	5	404004	13	NULL	NULL	0	NULL	body mass index-matched healthy controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A cross-sectional study involving 13 women with PCOS and 13 age - and body mass index-matched healthy controls was performed .
	manualset3
120017	1	404005	13	NULL	NULL	0	NULL	Oestradiol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Oestradiol decreases the activity of mRNA encoding the alpha and beta subunits of gonadotrophins .
	manualset3
120018	2	404005	13	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Oestradiol decreases the activity of mRNA encoding the alpha and beta subunits of gonadotrophins .
	manualset3
120019	3	404005	13	NULL	NULL	0	NULL	mRNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Oestradiol decreases the activity of mRNA encoding the alpha and beta subunits of gonadotrophins .
	manualset3
120020	4	404005	13	NULL	NULL	0	NULL	alpha subunit of gonadotrophins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Oestradiol decreases the activity of mRNA encoding the alpha and beta subunits of gonadotrophins .
	manualset3
120021	5	404005	13	NULL	NULL	0	NULL	beta subunit of gonadotrophins 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Oestradiol decreases the activity of mRNA encoding the alpha and beta subunits of gonadotrophins .
	manualset3
120022	1	404006	13	NULL	NULL	0	NULL	Oestrogen 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Oestrogen priming increases the LH and FSH response to LH-RH to a smaller degree in ovariectomized , lactating , than in non-lactating , ovariectomized rats .
	manualset3
120023	2	404006	13	NULL	NULL	0	NULL	LH response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Oestrogen priming increases the LH and FSH response to LH-RH to a smaller degree in ovariectomized , lactating , than in non-lactating , ovariectomized rats .
	manualset3
120024	3	404006	13	NULL	NULL	0	NULL	FSH response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Oestrogen priming increases the LH and FSH response to LH-RH to a smaller degree in ovariectomized , lactating , than in non-lactating , ovariectomized rats .
	manualset3
120025	4	404006	13	NULL	NULL	0	NULL	LH-RH	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Oestrogen priming increases the LH and FSH response to LH-RH to a smaller degree in ovariectomized , lactating , than in non-lactating , ovariectomized rats .
	manualset3
120026	5	404006	13	NULL	NULL	0	NULL	smaller degree 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Oestrogen priming increases the LH and FSH response to LH-RH to a smaller degree in ovariectomized , lactating , than in non-lactating , ovariectomized rats .
	manualset3
120027	6	404006	13	NULL	NULL	0	NULL	ovariectomized, lactating  rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Oestrogen priming increases the LH and FSH response to LH-RH to a smaller degree in ovariectomized , lactating , than in non-lactating , ovariectomized rats .
	manualset3
120028	7	404006	13	NULL	NULL	0	NULL	non-lactating , ovariectomized rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Oestrogen priming increases the LH and FSH response to LH-RH to a smaller degree in ovariectomized , lactating , than in non-lactating , ovariectomized rats .
	manualset3
120029	1	404007	13	NULL	NULL	0	NULL	1076 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 1076 patients with intracranial ruptured aneurysms ( RA ) , 948 had the RA verified by angiography , and of 908 RA with a maximum diameter less than 25 mm , 162 RA were & lt ; 5 mm , 474 were between 5-10 mm and 272 were between 11-24 mm .
	manualset3
120030	2	404007	13	NULL	NULL	0	NULL	 intracranial ruptured aneurysms ( RA ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 1076 patients with intracranial ruptured aneurysms ( RA ) , 948 had the RA verified by angiography , and of 908 RA with a maximum diameter less than 25 mm , 162 RA were & lt ; 5 mm , 474 were between 5-10 mm and 272 were between 11-24 mm .
	manualset3
120031	3	404007	13	NULL	NULL	0	NULL	948	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 1076 patients with intracranial ruptured aneurysms ( RA ) , 948 had the RA verified by angiography , and of 908 RA with a maximum diameter less than 25 mm , 162 RA were & lt ; 5 mm , 474 were between 5-10 mm and 272 were between 11-24 mm .
	manualset3
120032	4	404007	13	NULL	NULL	0	NULL	RA	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 1076 patients with intracranial ruptured aneurysms ( RA ) , 948 had the RA verified by angiography , and of 908 RA with a maximum diameter less than 25 mm , 162 RA were & lt ; 5 mm , 474 were between 5-10 mm and 272 were between 11-24 mm .
	manualset3
120033	5	404007	13	NULL	NULL	0	NULL	angiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 1076 patients with intracranial ruptured aneurysms ( RA ) , 948 had the RA verified by angiography , and of 908 RA with a maximum diameter less than 25 mm , 162 RA were & lt ; 5 mm , 474 were between 5-10 mm and 272 were between 11-24 mm .
	manualset3
120034	6	404007	13	NULL	NULL	NULL	NULL	908 RA	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Of 1076 patients with intracranial ruptured aneurysms ( RA ) , 948 had the RA verified by angiography , and of 908 RA with a maximum diameter less than 25 mm , 162 RA were & lt ; 5 mm , 474 were between 5-10 mm and 272 were between 11-24 mm .
	manualset3
120035	7	404007	13	NULL	NULL	0	NULL	diameter	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 1076 patients with intracranial ruptured aneurysms ( RA ) , 948 had the RA verified by angiography , and of 908 RA with a maximum diameter less than 25 mm , 162 RA were & lt ; 5 mm , 474 were between 5-10 mm and 272 were between 11-24 mm .
	manualset3
120036	8	404007	13	NULL	NULL	0	NULL	25 mm 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 1076 patients with intracranial ruptured aneurysms ( RA ) , 948 had the RA verified by angiography , and of 908 RA with a maximum diameter less than 25 mm , 162 RA were & lt ; 5 mm , 474 were between 5-10 mm and 272 were between 11-24 mm .
	manualset3
120037	9	404007	13	NULL	NULL	0	NULL	162 RA	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 1076 patients with intracranial ruptured aneurysms ( RA ) , 948 had the RA verified by angiography , and of 908 RA with a maximum diameter less than 25 mm , 162 RA were & lt ; 5 mm , 474 were between 5-10 mm and 272 were between 11-24 mm .
	manualset3
120038	10	404007	13	NULL	NULL	0	NULL	5 mm 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 1076 patients with intracranial ruptured aneurysms ( RA ) , 948 had the RA verified by angiography , and of 908 RA with a maximum diameter less than 25 mm , 162 RA were & lt ; 5 mm , 474 were between 5-10 mm and 272 were between 11-24 mm .
	manualset3
120039	11	404007	13	NULL	NULL	NULL	NULL	474	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Of 1076 patients with intracranial ruptured aneurysms ( RA ) , 948 had the RA verified by angiography , and of 908 RA with a maximum diameter less than 25 mm , 162 RA were & lt ; 5 mm , 474 were between 5-10 mm and 272 were between 11-24 mm .
	manualset3
120040	12	404007	13	NULL	NULL	0	NULL	5-10 mm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 1076 patients with intracranial ruptured aneurysms ( RA ) , 948 had the RA verified by angiography , and of 908 RA with a maximum diameter less than 25 mm , 162 RA were & lt ; 5 mm , 474 were between 5-10 mm and 272 were between 11-24 mm .
	manualset3
120041	13	404007	13	NULL	NULL	NULL	NULL	272	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Of 1076 patients with intracranial ruptured aneurysms ( RA ) , 948 had the RA verified by angiography , and of 908 RA with a maximum diameter less than 25 mm , 162 RA were & lt ; 5 mm , 474 were between 5-10 mm and 272 were between 11-24 mm .
	manualset3
120043	14	404007	13	NULL	NULL	0	NULL	11-24 mm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 1076 patients with intracranial ruptured aneurysms ( RA ) , 948 had the RA verified by angiography , and of 908 RA with a maximum diameter less than 25 mm , 162 RA were & lt ; 5 mm , 474 were between 5-10 mm and 272 were between 11-24 mm .
	manualset3
120044	1	404008	13	NULL	NULL	0	NULL	16 evaluable patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 16 evaluable patients with breast cancer , 15 responded ( six complete responses ) .
	manualset3
120046	2	404008	13	NULL	NULL	0	NULL	 breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 16 evaluable patients with breast cancer , 15 responded ( six complete responses ) .
	manualset3
120047	3	404008	13	NULL	NULL	0	NULL	15	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 16 evaluable patients with breast cancer , 15 responded ( six complete responses ) .
	manualset3
120048	4	404008	13	NULL	NULL	0	NULL	six complete responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 16 evaluable patients with breast cancer , 15 responded ( six complete responses ) .
	manualset3
120054	1	404009	13	NULL	NULL	0	NULL	167 sera	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 167 sera from humans infected with P. falciparum but not P. malariae , 133 ( 79.6 % ) reacted with RESA ; of these , 43 ( 25.7 % of the total ) reacted with PEMA but not RESA .
	manualset3
120055	2	404009	13	NULL	NULL	0	NULL	humans	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 167 sera from humans infected with P. falciparum but not P. malariae , 133 ( 79.6 % ) reacted with RESA ; of these , 43 ( 25.7 % of the total ) reacted with PEMA but not RESA .
	manualset3
120056	3	404009	13	NULL	NULL	0	NULL	P. falciparum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 167 sera from humans infected with P. falciparum but not P. malariae , 133 ( 79.6 % ) reacted with RESA ; of these , 43 ( 25.7 % of the total ) reacted with PEMA but not RESA .
	manualset3
120057	4	404009	13	NULL	NULL	0	NULL	P. malariae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 167 sera from humans infected with P. falciparum but not P. malariae , 133 ( 79.6 % ) reacted with RESA ; of these , 43 ( 25.7 % of the total ) reacted with PEMA but not RESA .
	manualset3
120058	5	404009	13	NULL	NULL	0	NULL	133 ( 79.6 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 167 sera from humans infected with P. falciparum but not P. malariae , 133 ( 79.6 % ) reacted with RESA ; of these , 43 ( 25.7 % of the total ) reacted with PEMA but not RESA .
	manualset3
120059	6	404009	13	NULL	NULL	0	NULL	RESA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 167 sera from humans infected with P. falciparum but not P. malariae , 133 ( 79.6 % ) reacted with RESA ; of these , 43 ( 25.7 % of the total ) reacted with PEMA but not RESA .
	manualset3
120060	7	404009	13	NULL	NULL	0	NULL	43 ( 25.7 % of the total )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 167 sera from humans infected with P. falciparum but not P. malariae , 133 ( 79.6 % ) reacted with RESA ; of these , 43 ( 25.7 % of the total ) reacted with PEMA but not RESA .
	manualset3
120061	8	404009	13	NULL	NULL	0	NULL	PEMA 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 167 sera from humans infected with P. falciparum but not P. malariae , 133 ( 79.6 % ) reacted with RESA ; of these , 43 ( 25.7 % of the total ) reacted with PEMA but not RESA .
	manualset3
120062	9	404009	13	NULL	NULL	0	NULL	RESA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 167 sera from humans infected with P. falciparum but not P. malariae , 133 ( 79.6 % ) reacted with RESA ; of these , 43 ( 25.7 % of the total ) reacted with PEMA but not RESA .
	manualset3
120065	1	404010	13	NULL	NULL	0	NULL	cross-sectional study 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A cross-sectional study of medication-related factors and caries experience in asthmatic children .
	manualset3
120066	2	404010	13	NULL	NULL	0	NULL	medication-related factors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A cross-sectional study of medication-related factors and caries experience in asthmatic children .
	manualset3
120069	3	404010	13	NULL	NULL	0	NULL	caries experience	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A cross-sectional study of medication-related factors and caries experience in asthmatic children .
	manualset3
120070	4	404010	13	NULL	NULL	0	NULL	asthmatic children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A cross-sectional study of medication-related factors and caries experience in asthmatic children .
	manualset3
120073	1	404011	13	NULL	NULL	0	NULL	21 vaccinated participants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 21 vaccinated participants with baseline serologic testing , 14 ( 67 % ) were reactive to measles , 19 ( 91 % ) to mumps , and 20 ( 95 % ) to rubella .
	manualset3
120076	2	404011	13	NULL	NULL	0	NULL	baseline serologic testing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 21 vaccinated participants with baseline serologic testing , 14 ( 67 % ) were reactive to measles , 19 ( 91 % ) to mumps , and 20 ( 95 % ) to rubella .
	manualset3
120077	3	404011	13	NULL	NULL	0	NULL	14 ( 67 % ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 21 vaccinated participants with baseline serologic testing , 14 ( 67 % ) were reactive to measles , 19 ( 91 % ) to mumps , and 20 ( 95 % ) to rubella .
	manualset3
120078	4	404011	13	NULL	NULL	0	NULL	measles	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 21 vaccinated participants with baseline serologic testing , 14 ( 67 % ) were reactive to measles , 19 ( 91 % ) to mumps , and 20 ( 95 % ) to rubella .
	manualset3
120079	5	404011	13	NULL	NULL	0	NULL	19 ( 91 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 21 vaccinated participants with baseline serologic testing , 14 ( 67 % ) were reactive to measles , 19 ( 91 % ) to mumps , and 20 ( 95 % ) to rubella .
	manualset3
120081	6	404011	13	NULL	NULL	0	NULL	mumps 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 21 vaccinated participants with baseline serologic testing , 14 ( 67 % ) were reactive to measles , 19 ( 91 % ) to mumps , and 20 ( 95 % ) to rubella .
	manualset3
120083	7	404011	13	NULL	NULL	0	NULL	20 ( 95 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 21 vaccinated participants with baseline serologic testing , 14 ( 67 % ) were reactive to measles , 19 ( 91 % ) to mumps , and 20 ( 95 % ) to rubella .
	manualset3
120084	8	404011	13	NULL	NULL	0	NULL	rubella 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 21 vaccinated participants with baseline serologic testing , 14 ( 67 % ) were reactive to measles , 19 ( 91 % ) to mumps , and 20 ( 95 % ) to rubella .
	manualset3
120086	1	404012	13	NULL	NULL	0	NULL	55 inbred strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 55 inbred strains , 52 expressed either Qed-1a or Qed-1b , which thus behaved as products of alleles of a single locus , Qed-1 .
	manualset3
120089	2	404012	13	NULL	NULL	0	NULL	52	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 55 inbred strains , 52 expressed either Qed-1a or Qed-1b , which thus behaved as products of alleles of a single locus , Qed-1 .
	manualset3
120090	3	404012	13	NULL	NULL	0	NULL	Qed-1a 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 55 inbred strains , 52 expressed either Qed-1a or Qed-1b , which thus behaved as products of alleles of a single locus , Qed-1 .
	manualset3
120091	4	404012	13	NULL	NULL	0	NULL	Qed-1b	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 55 inbred strains , 52 expressed either Qed-1a or Qed-1b , which thus behaved as products of alleles of a single locus , Qed-1 .
	manualset3
120094	5	404012	13	NULL	NULL	0	NULL	products	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 55 inbred strains , 52 expressed either Qed-1a or Qed-1b , which thus behaved as products of alleles of a single locus , Qed-1 .
	manualset3
120095	6	404012	13	NULL	NULL	0	NULL	alleles of a single locus	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 55 inbred strains , 52 expressed either Qed-1a or Qed-1b , which thus behaved as products of alleles of a single locus , Qed-1 .
	manualset3
120096	7	404012	13	NULL	NULL	0	NULL	Qed-1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 55 inbred strains , 52 expressed either Qed-1a or Qed-1b , which thus behaved as products of alleles of a single locus , Qed-1 .
	manualset3
120120	1	404013	13	NULL	NULL	0	NULL	611 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 611 patients with biopsy-proved adenocarcinoma of the prostate , spinal cord compression developed in 41 ( 6.7 % ) at a median interval of twenty-four months after primary diagnosis .
	manualset3
120121	2	404013	13	NULL	NULL	0	NULL	adenocarcinoma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 611 patients with biopsy-proved adenocarcinoma of the prostate , spinal cord compression developed in 41 ( 6.7 % ) at a median interval of twenty-four months after primary diagnosis .
	manualset3
120122	3	404013	13	NULL	NULL	0	NULL	prostate 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 611 patients with biopsy-proved adenocarcinoma of the prostate , spinal cord compression developed in 41 ( 6.7 % ) at a median interval of twenty-four months after primary diagnosis .
	manualset3
120123	4	404013	13	NULL	NULL	0	NULL	spinal cord compression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 611 patients with biopsy-proved adenocarcinoma of the prostate , spinal cord compression developed in 41 ( 6.7 % ) at a median interval of twenty-four months after primary diagnosis .
	manualset3
120125	5	404013	13	NULL	NULL	0	NULL	41 ( 6.7 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 611 patients with biopsy-proved adenocarcinoma of the prostate , spinal cord compression developed in 41 ( 6.7 % ) at a median interval of twenty-four months after primary diagnosis .
	manualset3
120127	6	404013	13	NULL	NULL	0	NULL	median interval	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 611 patients with biopsy-proved adenocarcinoma of the prostate , spinal cord compression developed in 41 ( 6.7 % ) at a median interval of twenty-four months after primary diagnosis .
	manualset3
120128	7	404013	13	NULL	NULL	0	NULL	twenty-four months 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 611 patients with biopsy-proved adenocarcinoma of the prostate , spinal cord compression developed in 41 ( 6.7 % ) at a median interval of twenty-four months after primary diagnosis .
	manualset3
120130	8	404013	13	NULL	NULL	0	NULL	primary diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 611 patients with biopsy-proved adenocarcinoma of the prostate , spinal cord compression developed in 41 ( 6.7 % ) at a median interval of twenty-four months after primary diagnosis .
	manualset3
120142	1	404014	13	NULL	NULL	0	NULL	crucial event	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A crucial event in tumor progression referred to as epithelial to mesenchymal transition ( EMT ) allows carcinoma cells to acquire invasive properties .
	manualset3
120144	2	404014	13	NULL	NULL	0	NULL	tumor progression 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A crucial event in tumor progression referred to as epithelial to mesenchymal transition ( EMT ) allows carcinoma cells to acquire invasive properties .
	manualset3
120145	3	404014	13	NULL	NULL	0	NULL	epithelial to mesenchymal transition ( EMT )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A crucial event in tumor progression referred to as epithelial to mesenchymal transition ( EMT ) allows carcinoma cells to acquire invasive properties .
	manualset3
120146	4	404014	13	NULL	NULL	0	NULL	carcinoma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A crucial event in tumor progression referred to as epithelial to mesenchymal transition ( EMT ) allows carcinoma cells to acquire invasive properties .
	manualset3
120148	5	404014	13	NULL	NULL	0	NULL	invasive properties 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A crucial event in tumor progression referred to as epithelial to mesenchymal transition ( EMT ) allows carcinoma cells to acquire invasive properties .
	manualset3
120152	1	404015	13	NULL	NULL	0	NULL	China 's	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Of China 's approximately 463 million women and men below age 20 in 1982 , 225 million are women who will turn 20 ( the minimum age for marriage under the 1982 Marriage Law ) during the next 2 decades .
	manualset3
120153	2	404015	13	NULL	NULL	0	NULL	463 million	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of China 's approximately 463 million women and men below age 20 in 1982 , 225 million are women who will turn 20 ( the minimum age for marriage under the 1982 Marriage Law ) during the next 2 decades .
	manualset3
120154	3	404015	13	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of China 's approximately 463 million women and men below age 20 in 1982 , 225 million are women who will turn 20 ( the minimum age for marriage under the 1982 Marriage Law ) during the next 2 decades .
	manualset3
120155	4	404015	13	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of China 's approximately 463 million women and men below age 20 in 1982 , 225 million are women who will turn 20 ( the minimum age for marriage under the 1982 Marriage Law ) during the next 2 decades .
	manualset3
120156	5	404015	13	NULL	NULL	0	NULL	age 20	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of China 's approximately 463 million women and men below age 20 in 1982 , 225 million are women who will turn 20 ( the minimum age for marriage under the 1982 Marriage Law ) during the next 2 decades .
	manualset3
120157	6	404015	13	NULL	NULL	0	NULL	1982	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Of China 's approximately 463 million women and men below age 20 in 1982 , 225 million are women who will turn 20 ( the minimum age for marriage under the 1982 Marriage Law ) during the next 2 decades .
	manualset3
120158	7	404015	13	NULL	NULL	0	NULL	225 million	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of China 's approximately 463 million women and men below age 20 in 1982 , 225 million are women who will turn 20 ( the minimum age for marriage under the 1982 Marriage Law ) during the next 2 decades .
	manualset3
120159	8	404015	13	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of China 's approximately 463 million women and men below age 20 in 1982 , 225 million are women who will turn 20 ( the minimum age for marriage under the 1982 Marriage Law ) during the next 2 decades .
	manualset3
120160	9	404015	13	NULL	NULL	0	NULL	20	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of China 's approximately 463 million women and men below age 20 in 1982 , 225 million are women who will turn 20 ( the minimum age for marriage under the 1982 Marriage Law ) during the next 2 decades .
	manualset3
120161	10	404015	13	NULL	NULL	0	NULL	minimum age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of China 's approximately 463 million women and men below age 20 in 1982 , 225 million are women who will turn 20 ( the minimum age for marriage under the 1982 Marriage Law ) during the next 2 decades .
	manualset3
120162	11	404015	13	NULL	NULL	0	NULL	marriage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Of China 's approximately 463 million women and men below age 20 in 1982 , 225 million are women who will turn 20 ( the minimum age for marriage under the 1982 Marriage Law ) during the next 2 decades .
	manualset3
120163	12	404015	13	NULL	NULL	0	NULL	1982 Marriage Law 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Of China 's approximately 463 million women and men below age 20 in 1982 , 225 million are women who will turn 20 ( the minimum age for marriage under the 1982 Marriage Law ) during the next 2 decades .
	manualset3
120164	13	404015	13	NULL	NULL	0	NULL	next 2 decades	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Of China 's approximately 463 million women and men below age 20 in 1982 , 225 million are women who will turn 20 ( the minimum age for marriage under the 1982 Marriage Law ) during the next 2 decades .
	manualset3
120165	1	404016	13	NULL	NULL	NULL	NULL	adipokines 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Of all adipokines investigated , multivariate logistic regression analysis showed that adiponectin was the exclusive predictor of the development of postoperative PVR after scleral buckling surgery ( P = 0.003 ) .
	manualset3
120166	2	404016	13	NULL	NULL	0	NULL	multivariate logistic regression analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of all adipokines investigated , multivariate logistic regression analysis showed that adiponectin was the exclusive predictor of the development of postoperative PVR after scleral buckling surgery ( P = 0.003 ) .
	manualset3
120167	3	404016	13	NULL	NULL	0	NULL	adiponectin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Of all adipokines investigated , multivariate logistic regression analysis showed that adiponectin was the exclusive predictor of the development of postoperative PVR after scleral buckling surgery ( P = 0.003 ) .
	manualset3
120168	4	404016	13	NULL	NULL	0	NULL	predictor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Of all adipokines investigated , multivariate logistic regression analysis showed that adiponectin was the exclusive predictor of the development of postoperative PVR after scleral buckling surgery ( P = 0.003 ) .
	manualset3
120169	5	404016	13	NULL	NULL	0	NULL	development 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of all adipokines investigated , multivariate logistic regression analysis showed that adiponectin was the exclusive predictor of the development of postoperative PVR after scleral buckling surgery ( P = 0.003 ) .
	manualset3
120170	6	404016	13	NULL	NULL	0	NULL	postoperative PVR	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of all adipokines investigated , multivariate logistic regression analysis showed that adiponectin was the exclusive predictor of the development of postoperative PVR after scleral buckling surgery ( P = 0.003 ) .
	manualset3
120171	7	404016	13	NULL	NULL	0	NULL	scleral buckling surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Of all adipokines investigated , multivariate logistic regression analysis showed that adiponectin was the exclusive predictor of the development of postoperative PVR after scleral buckling surgery ( P = 0.003 ) .
	manualset3
120172	8	404016	13	NULL	NULL	0	NULL	P = 0.003 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of all adipokines investigated , multivariate logistic regression analysis showed that adiponectin was the exclusive predictor of the development of postoperative PVR after scleral buckling surgery ( P = 0.003 ) .
	manualset3
120173	1	404017	13	NULL	NULL	0	NULL	coupling hypotheses	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Of all coupling hypotheses , only the parallel-coupling hypothesis can explain the observations , unless variation of the H + / ATP stoichiometry of the ATPase proton pump is accepted .
	manualset3
120174	2	404017	13	NULL	NULL	0	NULL	parallel-coupling hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Of all coupling hypotheses , only the parallel-coupling hypothesis can explain the observations , unless variation of the H + / ATP stoichiometry of the ATPase proton pump is accepted .
	manualset3
120175	3	404017	13	NULL	NULL	0	NULL	observations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Of all coupling hypotheses , only the parallel-coupling hypothesis can explain the observations , unless variation of the H + / ATP stoichiometry of the ATPase proton pump is accepted .
	manualset3
120176	4	404017	13	NULL	NULL	0	NULL	variation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Of all coupling hypotheses , only the parallel-coupling hypothesis can explain the observations , unless variation of the H + / ATP stoichiometry of the ATPase proton pump is accepted .
	manualset3
120177	5	404017	13	NULL	NULL	0	NULL	H + / ATP stoichiometry	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Of all coupling hypotheses , only the parallel-coupling hypothesis can explain the observations , unless variation of the H + / ATP stoichiometry of the ATPase proton pump is accepted .
	manualset3
120178	6	404017	13	NULL	NULL	0	NULL	ATPase proton pump 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Of all coupling hypotheses , only the parallel-coupling hypothesis can explain the observations , unless variation of the H + / ATP stoichiometry of the ATPase proton pump is accepted .
	manualset3
120179	1	404018	13	NULL	NULL	0	NULL	practical interest	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Of both practical and theoretical interest is the observation of a rapid collision-mediated homogeneous relaxation process that can return these large ions to the center of the cell within a few hundred milliseconds after excitation .
	manualset3
120180	2	404018	13	NULL	NULL	0	NULL	theoretical interest	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Of both practical and theoretical interest is the observation of a rapid collision-mediated homogeneous relaxation process that can return these large ions to the center of the cell within a few hundred milliseconds after excitation .
	manualset3
120181	3	404018	13	NULL	NULL	0	NULL	observation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Of both practical and theoretical interest is the observation of a rapid collision-mediated homogeneous relaxation process that can return these large ions to the center of the cell within a few hundred milliseconds after excitation .
	manualset3
120182	4	404018	13	NULL	NULL	NULL	NULL	relaxation process	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Of both practical and theoretical interest is the observation of a rapid collision-mediated homogeneous relaxation process that can return these large ions to the center of the cell within a few hundred milliseconds after excitation .
	manualset3
120183	5	404018	13	NULL	NULL	0	NULL	large ions 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Of both practical and theoretical interest is the observation of a rapid collision-mediated homogeneous relaxation process that can return these large ions to the center of the cell within a few hundred milliseconds after excitation .
	manualset3
120184	6	404018	13	NULL	NULL	0	NULL	center of the cell	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Of both practical and theoretical interest is the observation of a rapid collision-mediated homogeneous relaxation process that can return these large ions to the center of the cell within a few hundred milliseconds after excitation .
	manualset3
120185	7	404018	13	NULL	NULL	0	NULL	few hundred milliseconds	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Of both practical and theoretical interest is the observation of a rapid collision-mediated homogeneous relaxation process that can return these large ions to the center of the cell within a few hundred milliseconds after excitation .
	manualset3
120186	8	404018	13	NULL	NULL	0	NULL	excitation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Of both practical and theoretical interest is the observation of a rapid collision-mediated homogeneous relaxation process that can return these large ions to the center of the cell within a few hundred milliseconds after excitation .
	manualset3
120192	1	404019	13	NULL	NULL	0	NULL	clinical significance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of clinical significance is the fact that eight of 29 ( 27.6 % ) tumors changed from positive estrogen receptor values in the biopsy specimen to negative ( four ) and borderline ( four ) in the mastectomy specimens .
	manualset3
120195	2	404019	13	NULL	NULL	0	NULL	fact 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of clinical significance is the fact that eight of 29 ( 27.6 % ) tumors changed from positive estrogen receptor values in the biopsy specimen to negative ( four ) and borderline ( four ) in the mastectomy specimens .
	manualset3
120197	3	404019	13	NULL	NULL	NULL	NULL	eight of 29 ( 27.6 % )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Of clinical significance is the fact that eight of 29 ( 27.6 % ) tumors changed from positive estrogen receptor values in the biopsy specimen to negative ( four ) and borderline ( four ) in the mastectomy specimens .
	manualset3
120198	4	404019	13	NULL	NULL	0	NULL	positive estrogen receptor values	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of clinical significance is the fact that eight of 29 ( 27.6 % ) tumors changed from positive estrogen receptor values in the biopsy specimen to negative ( four ) and borderline ( four ) in the mastectomy specimens .
	manualset3
120199	5	404019	13	NULL	NULL	0	NULL	biopsy specimen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Of clinical significance is the fact that eight of 29 ( 27.6 % ) tumors changed from positive estrogen receptor values in the biopsy specimen to negative ( four ) and borderline ( four ) in the mastectomy specimens .
	manualset3
120200	6	404019	13	NULL	NULL	0	NULL	negative ( four )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of clinical significance is the fact that eight of 29 ( 27.6 % ) tumors changed from positive estrogen receptor values in the biopsy specimen to negative ( four ) and borderline ( four ) in the mastectomy specimens .
	manualset3
120201	7	404019	13	NULL	NULL	0	NULL	borderline ( four ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of clinical significance is the fact that eight of 29 ( 27.6 % ) tumors changed from positive estrogen receptor values in the biopsy specimen to negative ( four ) and borderline ( four ) in the mastectomy specimens .
	manualset3
120202	8	404019	13	NULL	NULL	0	NULL	mastectomy specimens	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Of clinical significance is the fact that eight of 29 ( 27.6 % ) tumors changed from positive estrogen receptor values in the biopsy specimen to negative ( four ) and borderline ( four ) in the mastectomy specimens .
	manualset3
121682	9	404019	13	NULL	NULL	0	NULL	tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of clinical significance is the fact that eight of 29 ( 27.6 % ) tumors changed from positive estrogen receptor values in the biopsy specimen to negative ( four ) and borderline ( four ) in the mastectomy specimens .
	manualset3
120203	1	404020	13	NULL	NULL	0	NULL	fifty cysts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of fifty cysts submitted to operation , twenty-one recurred in a mean period of seven months .
	manualset3
120204	2	404020	13	NULL	NULL	0	NULL	operation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Of fifty cysts submitted to operation , twenty-one recurred in a mean period of seven months .
	manualset3
120205	3	404020	13	NULL	NULL	0	NULL	twenty-one	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of fifty cysts submitted to operation , twenty-one recurred in a mean period of seven months .
	manualset3
120206	4	404020	13	NULL	NULL	0	NULL	mean period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Of fifty cysts submitted to operation , twenty-one recurred in a mean period of seven months .
	manualset3
120207	5	404020	13	NULL	NULL	0	NULL	seven months 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Of fifty cysts submitted to operation , twenty-one recurred in a mean period of seven months .
	manualset3
120208	1	404021	13	NULL	NULL	0	NULL	importance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Of great importance may be the damp proof improvement on medical equipment including anesthesia machines which have electronic circuits .
	manualset3
120209	2	404021	13	NULL	NULL	0	NULL	damp proof improvement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Of great importance may be the damp proof improvement on medical equipment including anesthesia machines which have electronic circuits .
	manualset3
120210	3	404021	13	NULL	NULL	0	NULL	medical equipment	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Of great importance may be the damp proof improvement on medical equipment including anesthesia machines which have electronic circuits .
	manualset3
120211	4	404021	13	NULL	NULL	0	NULL	anesthesia machines	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Of great importance may be the damp proof improvement on medical equipment including anesthesia machines which have electronic circuits .
	manualset3
120212	5	404021	13	NULL	NULL	0	NULL	electronic circuits	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Of great importance may be the damp proof improvement on medical equipment including anesthesia machines which have electronic circuits .
	manualset3
120217	1	404022	13	NULL	NULL	0	NULL	particular interest 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Of particular interest among the remainder are several membrane molecules that showed drastic differential expression , including , not surprisingly , the well-studied variant surface glycoproteins ( VSGs ) , invariant surface glycoproteins ( ISGs ) 65 and 75 , congolense epimastigote specific protein ( CESP ) , the surface protease GP63 , an amino acid transporter , a pteridine transporter and a haptoglobin-hemoglobin receptor .
	manualset3
120219	2	404022	13	NULL	NULL	0	NULL	several membrane molecules	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of particular interest among the remainder are several membrane molecules that showed drastic differential expression , including , not surprisingly , the well-studied variant surface glycoproteins ( VSGs ) , invariant surface glycoproteins ( ISGs ) 65 and 75 , congolense epimastigote specific protein ( CESP ) , the surface protease GP63 , an amino acid transporter , a pteridine transporter and a haptoglobin-hemoglobin receptor .
	manualset3
120221	3	404022	13	NULL	NULL	0	NULL	differential expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Of particular interest among the remainder are several membrane molecules that showed drastic differential expression , including , not surprisingly , the well-studied variant surface glycoproteins ( VSGs ) , invariant surface glycoproteins ( ISGs ) 65 and 75 , congolense epimastigote specific protein ( CESP ) , the surface protease GP63 , an amino acid transporter , a pteridine transporter and a haptoglobin-hemoglobin receptor .
	manualset3
120262	4	404022	13	NULL	NULL	0	NULL	variant surface glycoproteins ( VSGs )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of particular interest among the remainder are several membrane molecules that showed drastic differential expression , including , not surprisingly , the well-studied variant surface glycoproteins ( VSGs ) , invariant surface glycoproteins ( ISGs ) 65 and 75 , congolense epimastigote specific protein ( CESP ) , the surface protease GP63 , an amino acid transporter , a pteridine transporter and a haptoglobin-hemoglobin receptor .
	manualset3
120263	5	404022	13	NULL	NULL	0	NULL	invariant surface glycoproteins ( ISGs ) 65	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Of particular interest among the remainder are several membrane molecules that showed drastic differential expression , including , not surprisingly , the well-studied variant surface glycoproteins ( VSGs ) , invariant surface glycoproteins ( ISGs ) 65 and 75 , congolense epimastigote specific protein ( CESP ) , the surface protease GP63 , an amino acid transporter , a pteridine transporter and a haptoglobin-hemoglobin receptor .
	manualset3
120264	6	404022	13	NULL	NULL	0	NULL	invariant surface glycoproteins ( ISGs ) 75	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Of particular interest among the remainder are several membrane molecules that showed drastic differential expression , including , not surprisingly , the well-studied variant surface glycoproteins ( VSGs ) , invariant surface glycoproteins ( ISGs ) 65 and 75 , congolense epimastigote specific protein ( CESP ) , the surface protease GP63 , an amino acid transporter , a pteridine transporter and a haptoglobin-hemoglobin receptor .
	manualset3
120265	7	404022	13	NULL	NULL	0	NULL	congolense epimastigote specific protein ( CESP ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Of particular interest among the remainder are several membrane molecules that showed drastic differential expression , including , not surprisingly , the well-studied variant surface glycoproteins ( VSGs ) , invariant surface glycoproteins ( ISGs ) 65 and 75 , congolense epimastigote specific protein ( CESP ) , the surface protease GP63 , an amino acid transporter , a pteridine transporter and a haptoglobin-hemoglobin receptor .
	manualset3
120266	8	404022	13	NULL	NULL	0	NULL	surface protease GP63 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Of particular interest among the remainder are several membrane molecules that showed drastic differential expression , including , not surprisingly , the well-studied variant surface glycoproteins ( VSGs ) , invariant surface glycoproteins ( ISGs ) 65 and 75 , congolense epimastigote specific protein ( CESP ) , the surface protease GP63 , an amino acid transporter , a pteridine transporter and a haptoglobin-hemoglobin receptor .
	manualset3
120267	9	404022	13	NULL	NULL	0	NULL	pteridine transporter 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Of particular interest among the remainder are several membrane molecules that showed drastic differential expression , including , not surprisingly , the well-studied variant surface glycoproteins ( VSGs ) , invariant surface glycoproteins ( ISGs ) 65 and 75 , congolense epimastigote specific protein ( CESP ) , the surface protease GP63 , an amino acid transporter , a pteridine transporter and a haptoglobin-hemoglobin receptor .
	manualset3
120268	10	404022	13	NULL	NULL	0	NULL	 haptoglobin-hemoglobin receptor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Of particular interest among the remainder are several membrane molecules that showed drastic differential expression , including , not surprisingly , the well-studied variant surface glycoproteins ( VSGs ) , invariant surface glycoproteins ( ISGs ) 65 and 75 , congolense epimastigote specific protein ( CESP ) , the surface protease GP63 , an amino acid transporter , a pteridine transporter and a haptoglobin-hemoglobin receptor .
	manualset3
120269	1	404023	13	NULL	NULL	0	NULL	prime importance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of prime importance , Histosol is a safer and more efficient solvent for use in histological and pathological laboratories .
	manualset3
120270	2	404023	13	NULL	NULL	0	NULL	Histosol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Of prime importance , Histosol is a safer and more efficient solvent for use in histological and pathological laboratories .
	manualset3
120271	3	404023	13	NULL	NULL	0	NULL	efficient solvent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Of prime importance , Histosol is a safer and more efficient solvent for use in histological and pathological laboratories .
	manualset3
120272	4	404023	13	NULL	NULL	0	NULL	use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Of prime importance , Histosol is a safer and more efficient solvent for use in histological and pathological laboratories .
	manualset3
120273	5	404023	13	NULL	NULL	0	NULL	histological laboratories	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Of prime importance , Histosol is a safer and more efficient solvent for use in histological and pathological laboratories .
	manualset3
120274	6	404023	13	NULL	NULL	0	NULL	pathological laboratories	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Of prime importance , Histosol is a safer and more efficient solvent for use in histological and pathological laboratories .
	manualset3
120275	1	404024	13	NULL	NULL	0	NULL	145 episodes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 145 episodes of acute variceal bleeding 91.7 per cent were successfully controlled .
	manualset3
120276	2	404024	13	NULL	NULL	0	NULL	acute variceal bleeding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 145 episodes of acute variceal bleeding 91.7 per cent were successfully controlled .
	manualset3
120277	3	404024	13	NULL	NULL	0	NULL	91.7 per cent 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 145 episodes of acute variceal bleeding 91.7 per cent were successfully controlled .
	manualset3
120278	1	404025	13	NULL	NULL	0	NULL	200 elderly women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 200 elderly women invited to participate , 192 completed all interview questions .
	manualset3
120279	2	404025	13	NULL	NULL	0	NULL	192 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 200 elderly women invited to participate , 192 completed all interview questions .
	manualset3
120280	3	404025	13	NULL	NULL	0	NULL	interview questions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 200 elderly women invited to participate , 192 completed all interview questions .
	manualset3
120281	1	404026	13	NULL	NULL	0	NULL	22 control isolates	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 22 control isolates , 15 were S. epidermidis , and none had the special plasmid pattern nor any other recurring plasmid patterns .
	manualset3
120282	2	404026	13	NULL	NULL	0	NULL	15 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 22 control isolates , 15 were S. epidermidis , and none had the special plasmid pattern nor any other recurring plasmid patterns .
	manualset3
120283	3	404026	13	NULL	NULL	0	NULL	S. epidermidis 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 22 control isolates , 15 were S. epidermidis , and none had the special plasmid pattern nor any other recurring plasmid patterns .
	manualset3
120284	4	404026	13	NULL	NULL	0	NULL	special plasmid pattern	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 22 control isolates , 15 were S. epidermidis , and none had the special plasmid pattern nor any other recurring plasmid patterns .
	manualset3
120285	5	404026	13	NULL	NULL	0	NULL	plasmid patterns	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 22 control isolates , 15 were S. epidermidis , and none had the special plasmid pattern nor any other recurring plasmid patterns .
	manualset3
120286	1	404027	13	NULL	NULL	0	NULL	30 PTE subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 30 PTE subjects , thirteen who were rehabilitated by placement had more seizure disability ( p = 0.007 ) and a higher fertility rate ( p = 0.018 ) .
	manualset3
120287	2	404027	13	NULL	NULL	0	NULL	thirteen	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 30 PTE subjects , thirteen who were rehabilitated by placement had more seizure disability ( p = 0.007 ) and a higher fertility rate ( p = 0.018 ) .
	manualset3
120288	3	404027	13	NULL	NULL	0	NULL	placement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 30 PTE subjects , thirteen who were rehabilitated by placement had more seizure disability ( p = 0.007 ) and a higher fertility rate ( p = 0.018 ) .
	manualset3
120289	4	404027	13	NULL	NULL	0	NULL	seizure disability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 30 PTE subjects , thirteen who were rehabilitated by placement had more seizure disability ( p = 0.007 ) and a higher fertility rate ( p = 0.018 ) .
	manualset3
120290	5	404027	13	NULL	NULL	0	NULL	p = 0.007	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 30 PTE subjects , thirteen who were rehabilitated by placement had more seizure disability ( p = 0.007 ) and a higher fertility rate ( p = 0.018 ) .
	manualset3
120291	6	404027	13	NULL	NULL	0	NULL	 higher fertility rate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 30 PTE subjects , thirteen who were rehabilitated by placement had more seizure disability ( p = 0.007 ) and a higher fertility rate ( p = 0.018 ) .
	manualset3
120292	7	404027	13	NULL	NULL	0	NULL	p = 0.018 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 30 PTE subjects , thirteen who were rehabilitated by placement had more seizure disability ( p = 0.007 ) and a higher fertility rate ( p = 0.018 ) .
	manualset3
120293	1	404028	13	NULL	NULL	0	NULL	337 subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 337 subjects examined for knowledge about methods and means of transmission of brucellosis , 309 ( 92 % ) were ignorant while only 28 ( 8 % ) appeared to possess some knowledge as to the source , type of animal contact and presentation of illness .
	manualset3
120294	2	404028	13	NULL	NULL	0	NULL	knowledge	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 337 subjects examined for knowledge about methods and means of transmission of brucellosis , 309 ( 92 % ) were ignorant while only 28 ( 8 % ) appeared to possess some knowledge as to the source , type of animal contact and presentation of illness .
	manualset3
120295	3	404028	13	NULL	NULL	0	NULL	methods	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 337 subjects examined for knowledge about methods and means of transmission of brucellosis , 309 ( 92 % ) were ignorant while only 28 ( 8 % ) appeared to possess some knowledge as to the source , type of animal contact and presentation of illness .
	manualset3
120296	4	404028	13	NULL	NULL	0	NULL	means of transmission 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 337 subjects examined for knowledge about methods and means of transmission of brucellosis , 309 ( 92 % ) were ignorant while only 28 ( 8 % ) appeared to possess some knowledge as to the source , type of animal contact and presentation of illness .
	manualset3
120297	5	404028	13	NULL	NULL	0	NULL	brucellosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 337 subjects examined for knowledge about methods and means of transmission of brucellosis , 309 ( 92 % ) were ignorant while only 28 ( 8 % ) appeared to possess some knowledge as to the source , type of animal contact and presentation of illness .
	manualset3
120298	6	404028	13	NULL	NULL	0	NULL	309 ( 92 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 337 subjects examined for knowledge about methods and means of transmission of brucellosis , 309 ( 92 % ) were ignorant while only 28 ( 8 % ) appeared to possess some knowledge as to the source , type of animal contact and presentation of illness .
	manualset3
120299	7	404028	13	NULL	NULL	0	NULL	28 ( 8 % ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 337 subjects examined for knowledge about methods and means of transmission of brucellosis , 309 ( 92 % ) were ignorant while only 28 ( 8 % ) appeared to possess some knowledge as to the source , type of animal contact and presentation of illness .
	manualset3
120300	8	404028	13	NULL	NULL	0	NULL	knowledge	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 337 subjects examined for knowledge about methods and means of transmission of brucellosis , 309 ( 92 % ) were ignorant while only 28 ( 8 % ) appeared to possess some knowledge as to the source , type of animal contact and presentation of illness .
	manualset3
120301	9	404028	13	NULL	NULL	0	NULL	source	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 337 subjects examined for knowledge about methods and means of transmission of brucellosis , 309 ( 92 % ) were ignorant while only 28 ( 8 % ) appeared to possess some knowledge as to the source , type of animal contact and presentation of illness .
	manualset3
120302	10	404028	13	NULL	NULL	0	NULL	type of animal contact	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 337 subjects examined for knowledge about methods and means of transmission of brucellosis , 309 ( 92 % ) were ignorant while only 28 ( 8 % ) appeared to possess some knowledge as to the source , type of animal contact and presentation of illness .
	manualset3
120303	11	404028	13	NULL	NULL	0	NULL	presentation of illness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 337 subjects examined for knowledge about methods and means of transmission of brucellosis , 309 ( 92 % ) were ignorant while only 28 ( 8 % ) appeared to possess some knowledge as to the source , type of animal contact and presentation of illness .
	manualset3
120304	1	404029	13	NULL	NULL	0	NULL	497 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 497 patients identified , only 147 had been evaluated by a medical oncologist , and 82 of the 147 had received chemotherapy treatment , which is 16.5 % of the initial cohort .
	manualset3
120305	2	404029	13	NULL	NULL	0	NULL	147	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 497 patients identified , only 147 had been evaluated by a medical oncologist , and 82 of the 147 had received chemotherapy treatment , which is 16.5 % of the initial cohort .
	manualset3
120306	3	404029	13	NULL	NULL	0	NULL	medical oncologist 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 497 patients identified , only 147 had been evaluated by a medical oncologist , and 82 of the 147 had received chemotherapy treatment , which is 16.5 % of the initial cohort .
	manualset3
120307	4	404029	13	NULL	NULL	0	NULL	 82 of the 147 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 497 patients identified , only 147 had been evaluated by a medical oncologist , and 82 of the 147 had received chemotherapy treatment , which is 16.5 % of the initial cohort .
	manualset3
120308	5	404029	13	NULL	NULL	0	NULL	chemotherapy treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 497 patients identified , only 147 had been evaluated by a medical oncologist , and 82 of the 147 had received chemotherapy treatment , which is 16.5 % of the initial cohort .
	manualset3
120309	6	404029	13	NULL	NULL	0	NULL	16.5 % of the initial cohort 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 497 patients identified , only 147 had been evaluated by a medical oncologist , and 82 of the 147 had received chemotherapy treatment , which is 16.5 % of the initial cohort .
	manualset3
120310	1	404030	13	NULL	NULL	0	NULL	current ` explosion ' 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A current ` explosion ' of user groups does not imply that these form a homogeneous group , nor that they share similar perspectives .
	manualset3
120311	2	404030	13	NULL	NULL	0	NULL	user groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A current ` explosion ' of user groups does not imply that these form a homogeneous group , nor that they share similar perspectives .
	manualset3
120312	3	404030	13	NULL	NULL	0	NULL	form 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A current ` explosion ' of user groups does not imply that these form a homogeneous group , nor that they share similar perspectives .
	manualset3
120313	4	404030	13	NULL	NULL	0	NULL	homogeneous group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A current ` explosion ' of user groups does not imply that these form a homogeneous group , nor that they share similar perspectives .
	manualset3
120314	5	404030	13	NULL	NULL	0	NULL	perspectives	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A current ` explosion ' of user groups does not imply that these form a homogeneous group , nor that they share similar perspectives .
	manualset3
120332	1	404031	13	NULL	NULL	0	NULL	57 children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 57 children with rheumatic disorders of whom 25 had JRA , 4 ( 7 % ) reached a border zone , non-specific level of 1 : 64 by IFA , and 53 sera were non-reactive .
	manualset3
120333	2	404031	13	NULL	NULL	NULL	NULL	 rheumatic disorders 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Of the 57 children with rheumatic disorders of whom 25 had JRA , 4 ( 7 % ) reached a border zone , non-specific level of 1 : 64 by IFA , and 53 sera were non-reactive .
	manualset3
120334	3	404031	13	NULL	NULL	0	NULL	25	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 57 children with rheumatic disorders of whom 25 had JRA , 4 ( 7 % ) reached a border zone , non-specific level of 1 : 64 by IFA , and 53 sera were non-reactive .
	manualset3
120335	4	404031	13	NULL	NULL	NULL	NULL	JRA 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Of the 57 children with rheumatic disorders of whom 25 had JRA , 4 ( 7 % ) reached a border zone , non-specific level of 1 : 64 by IFA , and 53 sera were non-reactive .
	manualset3
120336	5	404031	13	NULL	NULL	0	NULL	4 ( 7 % ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 57 children with rheumatic disorders of whom 25 had JRA , 4 ( 7 % ) reached a border zone , non-specific level of 1 : 64 by IFA , and 53 sera were non-reactive .
	manualset3
120337	6	404031	13	NULL	NULL	0	NULL	border zone 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 57 children with rheumatic disorders of whom 25 had JRA , 4 ( 7 % ) reached a border zone , non-specific level of 1 : 64 by IFA , and 53 sera were non-reactive .
	manualset3
120338	7	404031	13	NULL	NULL	NULL	NULL	non-specific level	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Of the 57 children with rheumatic disorders of whom 25 had JRA , 4 ( 7 % ) reached a border zone , non-specific level of 1 : 64 by IFA , and 53 sera were non-reactive .
	manualset3
120339	8	404031	13	NULL	NULL	0	NULL	1 : 64	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 57 children with rheumatic disorders of whom 25 had JRA , 4 ( 7 % ) reached a border zone , non-specific level of 1 : 64 by IFA , and 53 sera were non-reactive .
	manualset3
120340	9	404031	13	NULL	NULL	0	NULL	IFA 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 57 children with rheumatic disorders of whom 25 had JRA , 4 ( 7 % ) reached a border zone , non-specific level of 1 : 64 by IFA , and 53 sera were non-reactive .
	manualset3
120341	10	404031	13	NULL	NULL	0	NULL	53 sera	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 57 children with rheumatic disorders of whom 25 had JRA , 4 ( 7 % ) reached a border zone , non-specific level of 1 : 64 by IFA , and 53 sera were non-reactive .
	manualset3
120342	1	404032	13	NULL	NULL	0	NULL	68 chimaeras	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 68 chimaeras in which the sex of both the donor and host component was established 62 proved to be fertile .
	manualset3
120343	2	404032	13	NULL	NULL	0	NULL	sex	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 68 chimaeras in which the sex of both the donor and host component was established 62 proved to be fertile .
	manualset3
120344	3	404032	13	NULL	NULL	0	NULL	donor	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 68 chimaeras in which the sex of both the donor and host component was established 62 proved to be fertile .
	manualset3
120345	4	404032	13	NULL	NULL	NULL	NULL	host component	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Of the 68 chimaeras in which the sex of both the donor and host component was established 62 proved to be fertile .
	manualset3
120346	5	404032	13	NULL	NULL	0	NULL	62	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 68 chimaeras in which the sex of both the donor and host component was established 62 proved to be fertile .
	manualset3
120347	1	404033	13	NULL	NULL	0	NULL	eight hybridomas 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the eight hybridomas secreting mAbs that react with human sperm , one , the Vic-1 antibody , was selected for detailed analysis because of its high degree of tissue specificity .
	manualset3
120348	2	404033	13	NULL	NULL	0	NULL	mAbs 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the eight hybridomas secreting mAbs that react with human sperm , one , the Vic-1 antibody , was selected for detailed analysis because of its high degree of tissue specificity .
	manualset3
120349	3	404033	13	NULL	NULL	0	NULL	human sperm	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the eight hybridomas secreting mAbs that react with human sperm , one , the Vic-1 antibody , was selected for detailed analysis because of its high degree of tissue specificity .
	manualset3
120350	4	404033	13	NULL	NULL	0	NULL	Vic-1 antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the eight hybridomas secreting mAbs that react with human sperm , one , the Vic-1 antibody , was selected for detailed analysis because of its high degree of tissue specificity .
	manualset3
120351	5	404033	13	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the eight hybridomas secreting mAbs that react with human sperm , one , the Vic-1 antibody , was selected for detailed analysis because of its high degree of tissue specificity .
	manualset3
120352	6	404033	13	NULL	NULL	0	NULL	high degree 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the eight hybridomas secreting mAbs that react with human sperm , one , the Vic-1 antibody , was selected for detailed analysis because of its high degree of tissue specificity .
	manualset3
120353	7	404033	13	NULL	NULL	0	NULL	tissue specificity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the eight hybridomas secreting mAbs that react with human sperm , one , the Vic-1 antibody , was selected for detailed analysis because of its high degree of tissue specificity .
	manualset3
120354	1	404034	13	NULL	NULL	0	NULL	physical map	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A cytogenetically based physical map of chromosome 1B in common wheat .
	manualset3
120355	2	404034	13	NULL	NULL	0	NULL	chromosome 1B 	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	A cytogenetically based physical map of chromosome 1B in common wheat .
	manualset3
120356	3	404034	13	NULL	NULL	0	NULL	wheat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A cytogenetically based physical map of chromosome 1B in common wheat .
	manualset3
120357	1	404035	13	NULL	NULL	0	NULL	etiologic factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the etiologic factors , smoking and Candida infection seemed to be correlated with the change of type .
	manualset3
120358	2	404035	13	NULL	NULL	0	NULL	Candida infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the etiologic factors , smoking and Candida infection seemed to be correlated with the change of type .
	manualset3
120359	3	404035	13	NULL	NULL	0	NULL	change of type	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the etiologic factors , smoking and Candida infection seemed to be correlated with the change of type .
	manualset3
125240	4	404035	13	NULL	NULL	0	NULL	smoking	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the etiologic factors , smoking and Candida infection seemed to be correlated with the change of type .
	manualset3
120360	1	404036	13	NULL	NULL	0	NULL	hypnotic agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the hypnotic agents currently under clinical investigation , so far only eszopiclone has been studied in regard to efficacy over a prolonged period ( 6 months ) with no evidence of significant tolerance .
	manualset3
120361	2	404036	13	NULL	NULL	0	NULL	clinical investigation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the hypnotic agents currently under clinical investigation , so far only eszopiclone has been studied in regard to efficacy over a prolonged period ( 6 months ) with no evidence of significant tolerance .
	manualset3
120362	3	404036	13	NULL	NULL	0	NULL	eszopiclone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the hypnotic agents currently under clinical investigation , so far only eszopiclone has been studied in regard to efficacy over a prolonged period ( 6 months ) with no evidence of significant tolerance .
	manualset3
120363	4	404036	13	NULL	NULL	0	NULL	efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the hypnotic agents currently under clinical investigation , so far only eszopiclone has been studied in regard to efficacy over a prolonged period ( 6 months ) with no evidence of significant tolerance .
	manualset3
120364	5	404036	13	NULL	NULL	0	NULL	regard	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the hypnotic agents currently under clinical investigation , so far only eszopiclone has been studied in regard to efficacy over a prolonged period ( 6 months ) with no evidence of significant tolerance .
	manualset3
120365	6	404036	13	NULL	NULL	0	NULL	period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the hypnotic agents currently under clinical investigation , so far only eszopiclone has been studied in regard to efficacy over a prolonged period ( 6 months ) with no evidence of significant tolerance .
	manualset3
120366	7	404036	13	NULL	NULL	0	NULL	6 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the hypnotic agents currently under clinical investigation , so far only eszopiclone has been studied in regard to efficacy over a prolonged period ( 6 months ) with no evidence of significant tolerance .
	manualset3
120367	8	404036	13	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the hypnotic agents currently under clinical investigation , so far only eszopiclone has been studied in regard to efficacy over a prolonged period ( 6 months ) with no evidence of significant tolerance .
	manualset3
120368	9	404036	13	NULL	NULL	0	NULL	significant tolerance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the hypnotic agents currently under clinical investigation , so far only eszopiclone has been studied in regard to efficacy over a prolonged period ( 6 months ) with no evidence of significant tolerance .
	manualset3
120369	1	404037	13	NULL	NULL	0	NULL	inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the inhibitors tested , 2 , 4-dinitrophenol , hydroxylamine and salicylaldoxime have no effect on light enhanced allagochrome and chlorogenic acid values except at high concentrations ( which are generally deleterious to leaf tissues and cause decreased values for both dark and light incubated samples ) .
	manualset3
120370	2	404037	13	NULL	NULL	0	NULL	2 , 4-dinitrophenol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the inhibitors tested , 2 , 4-dinitrophenol , hydroxylamine and salicylaldoxime have no effect on light enhanced allagochrome and chlorogenic acid values except at high concentrations ( which are generally deleterious to leaf tissues and cause decreased values for both dark and light incubated samples ) .
	manualset3
120371	3	404037	13	NULL	NULL	0	NULL	hydroxylamine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the inhibitors tested , 2 , 4-dinitrophenol , hydroxylamine and salicylaldoxime have no effect on light enhanced allagochrome and chlorogenic acid values except at high concentrations ( which are generally deleterious to leaf tissues and cause decreased values for both dark and light incubated samples ) .
	manualset3
120372	4	404037	13	NULL	NULL	0	NULL	salicylaldoxime 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the inhibitors tested , 2 , 4-dinitrophenol , hydroxylamine and salicylaldoxime have no effect on light enhanced allagochrome and chlorogenic acid values except at high concentrations ( which are generally deleterious to leaf tissues and cause decreased values for both dark and light incubated samples ) .
	manualset3
120373	5	404037	13	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the inhibitors tested , 2 , 4-dinitrophenol , hydroxylamine and salicylaldoxime have no effect on light enhanced allagochrome and chlorogenic acid values except at high concentrations ( which are generally deleterious to leaf tissues and cause decreased values for both dark and light incubated samples ) .
	manualset3
120374	6	404037	13	NULL	NULL	0	NULL	light	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the inhibitors tested , 2 , 4-dinitrophenol , hydroxylamine and salicylaldoxime have no effect on light enhanced allagochrome and chlorogenic acid values except at high concentrations ( which are generally deleterious to leaf tissues and cause decreased values for both dark and light incubated samples ) .
	manualset3
120375	7	404037	13	NULL	NULL	0	NULL	allagochrome	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the inhibitors tested , 2 , 4-dinitrophenol , hydroxylamine and salicylaldoxime have no effect on light enhanced allagochrome and chlorogenic acid values except at high concentrations ( which are generally deleterious to leaf tissues and cause decreased values for both dark and light incubated samples ) .
	manualset3
120376	8	404037	13	NULL	NULL	0	NULL	chlorogenic acid values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the inhibitors tested , 2 , 4-dinitrophenol , hydroxylamine and salicylaldoxime have no effect on light enhanced allagochrome and chlorogenic acid values except at high concentrations ( which are generally deleterious to leaf tissues and cause decreased values for both dark and light incubated samples ) .
	manualset3
120377	9	404037	13	NULL	NULL	0	NULL	high concentrations 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the inhibitors tested , 2 , 4-dinitrophenol , hydroxylamine and salicylaldoxime have no effect on light enhanced allagochrome and chlorogenic acid values except at high concentrations ( which are generally deleterious to leaf tissues and cause decreased values for both dark and light incubated samples ) .
	manualset3
120378	10	404037	13	NULL	NULL	0	NULL	leaf tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the inhibitors tested , 2 , 4-dinitrophenol , hydroxylamine and salicylaldoxime have no effect on light enhanced allagochrome and chlorogenic acid values except at high concentrations ( which are generally deleterious to leaf tissues and cause decreased values for both dark and light incubated samples ) .
	manualset3
120379	11	404037	13	NULL	NULL	0	NULL	 cause	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the inhibitors tested , 2 , 4-dinitrophenol , hydroxylamine and salicylaldoxime have no effect on light enhanced allagochrome and chlorogenic acid values except at high concentrations ( which are generally deleterious to leaf tissues and cause decreased values for both dark and light incubated samples ) .
	manualset3
120380	12	404037	13	NULL	NULL	0	NULL	values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the inhibitors tested , 2 , 4-dinitrophenol , hydroxylamine and salicylaldoxime have no effect on light enhanced allagochrome and chlorogenic acid values except at high concentrations ( which are generally deleterious to leaf tissues and cause decreased values for both dark and light incubated samples ) .
	manualset3
120381	13	404037	13	NULL	NULL	0	NULL	dark incubated samples	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the inhibitors tested , 2 , 4-dinitrophenol , hydroxylamine and salicylaldoxime have no effect on light enhanced allagochrome and chlorogenic acid values except at high concentrations ( which are generally deleterious to leaf tissues and cause decreased values for both dark and light incubated samples ) .
	manualset3
120382	14	404037	13	NULL	NULL	0	NULL	 light incubated samples 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the inhibitors tested , 2 , 4-dinitrophenol , hydroxylamine and salicylaldoxime have no effect on light enhanced allagochrome and chlorogenic acid values except at high concentrations ( which are generally deleterious to leaf tissues and cause decreased values for both dark and light incubated samples ) .
	manualset3
120383	1	404038	13	NULL	NULL	0	NULL	metabolites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the metabolites tested , glutamate and glutamine were the most effective for the generation of ATP .
	manualset3
120384	2	404038	13	NULL	NULL	0	NULL	glutamate 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the metabolites tested , glutamate and glutamine were the most effective for the generation of ATP .
	manualset3
120385	3	404038	13	NULL	NULL	0	NULL	glutamine 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the metabolites tested , glutamate and glutamine were the most effective for the generation of ATP .
	manualset3
120386	4	404038	13	NULL	NULL	NULL	NULL	generation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Of the metabolites tested , glutamate and glutamine were the most effective for the generation of ATP .
	manualset3
120387	5	404038	13	NULL	NULL	0	NULL	ATP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the metabolites tested , glutamate and glutamine were the most effective for the generation of ATP .
	manualset3
120388	1	404039	13	NULL	NULL	0	NULL	motor items	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the motor items , eating and grooming were easiest whereas stair climbing , tub/shower transfers and locomotion were most difficult .
	manualset3
120389	2	404039	13	NULL	NULL	0	NULL	stair	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the motor items , eating and grooming were easiest whereas stair climbing , tub/shower transfers and locomotion were most difficult .
	manualset3
120390	3	404039	13	NULL	NULL	0	NULL	tub/shower 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the motor items , eating and grooming were easiest whereas stair climbing , tub/shower transfers and locomotion were most difficult .
	manualset3
120391	4	404039	13	NULL	NULL	0	NULL	transfers	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the motor items , eating and grooming were easiest whereas stair climbing , tub/shower transfers and locomotion were most difficult .
	manualset3
120392	5	404039	13	NULL	NULL	0	NULL	locomotion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the motor items , eating and grooming were easiest whereas stair climbing , tub/shower transfers and locomotion were most difficult .
	manualset3
120393	1	404040	13	NULL	NULL	0	NULL	10 dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the remaining 10 dogs , clinical signs associated with hyperadrenocorticism resolved in the 7 dogs that had adrenocortical adenoma and in 1 of the 3 dogs that had carcinoma .
	manualset3
120394	2	404040	13	NULL	NULL	0	NULL	clinical signs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the remaining 10 dogs , clinical signs associated with hyperadrenocorticism resolved in the 7 dogs that had adrenocortical adenoma and in 1 of the 3 dogs that had carcinoma .
	manualset3
120395	3	404040	13	NULL	NULL	0	NULL	hyperadrenocorticism 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the remaining 10 dogs , clinical signs associated with hyperadrenocorticism resolved in the 7 dogs that had adrenocortical adenoma and in 1 of the 3 dogs that had carcinoma .
	manualset3
120396	4	404040	13	NULL	NULL	0	NULL	7 dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the remaining 10 dogs , clinical signs associated with hyperadrenocorticism resolved in the 7 dogs that had adrenocortical adenoma and in 1 of the 3 dogs that had carcinoma .
	manualset3
120397	5	404040	13	NULL	NULL	0	NULL	adrenocortical adenoma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the remaining 10 dogs , clinical signs associated with hyperadrenocorticism resolved in the 7 dogs that had adrenocortical adenoma and in 1 of the 3 dogs that had carcinoma .
	manualset3
120398	6	404040	13	NULL	NULL	0	NULL	1 of the 3 dogs 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the remaining 10 dogs , clinical signs associated with hyperadrenocorticism resolved in the 7 dogs that had adrenocortical adenoma and in 1 of the 3 dogs that had carcinoma .
	manualset3
120399	7	404040	13	NULL	NULL	0	NULL	carcinoma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the remaining 10 dogs , clinical signs associated with hyperadrenocorticism resolved in the 7 dogs that had adrenocortical adenoma and in 1 of the 3 dogs that had carcinoma .
	manualset3
120400	1	404041	13	NULL	NULL	0	NULL	five sera 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the remaining five sera , four were labeled `` too weak for typing '' and one `` HTLV of uncertain type '' by the program .
	manualset3
120401	2	404041	13	NULL	NULL	0	NULL	 four	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the remaining five sera , four were labeled `` too weak for typing '' and one `` HTLV of uncertain type '' by the program .
	manualset3
120402	3	404041	13	NULL	NULL	0	NULL	typing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the remaining five sera , four were labeled `` too weak for typing '' and one `` HTLV of uncertain type '' by the program .
	manualset3
120403	4	404041	13	NULL	NULL	0	NULL	HTLV of uncertain type	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the remaining five sera , four were labeled `` too weak for typing '' and one `` HTLV of uncertain type '' by the program .
	manualset3
120404	5	404041	13	NULL	NULL	0	NULL	program 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the remaining five sera , four were labeled `` too weak for typing '' and one `` HTLV of uncertain type '' by the program .
	manualset3
120405	1	404042	13	NULL	NULL	0	NULL	clones	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the sequenced clones , 29 matched with silkbase entries and these identified putative genes were classified into six functional groups such as regulatory , food utilization , stress response , metabolic , ribosomal and transposable elements .
	manualset3
120406	2	404042	13	NULL	NULL	0	NULL	29	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the sequenced clones , 29 matched with silkbase entries and these identified putative genes were classified into six functional groups such as regulatory , food utilization , stress response , metabolic , ribosomal and transposable elements .
	manualset3
120407	3	404042	13	NULL	NULL	0	NULL	silkbase entries 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the sequenced clones , 29 matched with silkbase entries and these identified putative genes were classified into six functional groups such as regulatory , food utilization , stress response , metabolic , ribosomal and transposable elements .
	manualset3
120408	4	404042	13	NULL	NULL	0	NULL	putative genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the sequenced clones , 29 matched with silkbase entries and these identified putative genes were classified into six functional groups such as regulatory , food utilization , stress response , metabolic , ribosomal and transposable elements .
	manualset3
120409	5	404042	13	NULL	NULL	0	NULL	six functional groups	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the sequenced clones , 29 matched with silkbase entries and these identified putative genes were classified into six functional groups such as regulatory , food utilization , stress response , metabolic , ribosomal and transposable elements .
	manualset3
120410	6	404042	13	NULL	NULL	0	NULL	regulatory elements	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the sequenced clones , 29 matched with silkbase entries and these identified putative genes were classified into six functional groups such as regulatory , food utilization , stress response , metabolic , ribosomal and transposable elements .
	manualset3
120411	7	404042	13	NULL	NULL	0	NULL	 food utilization elements	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the sequenced clones , 29 matched with silkbase entries and these identified putative genes were classified into six functional groups such as regulatory , food utilization , stress response , metabolic , ribosomal and transposable elements .
	manualset3
120412	8	404042	13	NULL	NULL	0	NULL	stress response elements	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the sequenced clones , 29 matched with silkbase entries and these identified putative genes were classified into six functional groups such as regulatory , food utilization , stress response , metabolic , ribosomal and transposable elements .
	manualset3
120413	9	404042	13	NULL	NULL	0	NULL	metabolic elements	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the sequenced clones , 29 matched with silkbase entries and these identified putative genes were classified into six functional groups such as regulatory , food utilization , stress response , metabolic , ribosomal and transposable elements .
	manualset3
120414	10	404042	13	NULL	NULL	0	NULL	ribosomal elements 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the sequenced clones , 29 matched with silkbase entries and these identified putative genes were classified into six functional groups such as regulatory , food utilization , stress response , metabolic , ribosomal and transposable elements .
	manualset3
120415	11	404042	13	NULL	NULL	0	NULL	transposable elements 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the sequenced clones , 29 matched with silkbase entries and these identified putative genes were classified into six functional groups such as regulatory , food utilization , stress response , metabolic , ribosomal and transposable elements .
	manualset3
120416	1	404043	13	NULL	NULL	0	NULL	three subgroups	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the three subgroups of localized scleroderma , patients with generalized morphoea had the highest levels of serum sCD23 .
	manualset3
120417	2	404043	13	NULL	NULL	0	NULL	localized scleroderma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the three subgroups of localized scleroderma , patients with generalized morphoea had the highest levels of serum sCD23 .
	manualset3
120418	3	404043	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the three subgroups of localized scleroderma , patients with generalized morphoea had the highest levels of serum sCD23 .
	manualset3
120419	4	404043	13	NULL	NULL	0	NULL	generalized morphoea	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the three subgroups of localized scleroderma , patients with generalized morphoea had the highest levels of serum sCD23 .
	manualset3
120420	5	404043	13	NULL	NULL	0	NULL	levels 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the three subgroups of localized scleroderma , patients with generalized morphoea had the highest levels of serum sCD23 .
	manualset3
120421	6	404043	13	NULL	NULL	0	NULL	serum sCD23 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the three subgroups of localized scleroderma , patients with generalized morphoea had the highest levels of serum sCD23 .
	manualset3
120422	1	404044	13	NULL	NULL	0	NULL	70 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of these , 70 % worked over 30 hours/week and half had flexible hours .
	manualset3
120423	2	404044	13	NULL	NULL	0	NULL	30 hours/week	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Of these , 70 % worked over 30 hours/week and half had flexible hours .
	manualset3
120424	3	404044	13	NULL	NULL	0	NULL	half 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of these , 70 % worked over 30 hours/week and half had flexible hours .
	manualset3
120425	4	404044	13	NULL	NULL	0	NULL	flexible hours	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Of these , 70 % worked over 30 hours/week and half had flexible hours .
	manualset3
120426	1	404045	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of these patients , 76 ( 6.8 % ) were diagnosed with DIC .
	manualset3
120427	2	404045	13	NULL	NULL	0	NULL	76 ( 6.8 % ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of these patients , 76 ( 6.8 % ) were diagnosed with DIC .
	manualset3
120428	3	404045	13	NULL	NULL	0	NULL	DIC	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of these patients , 76 ( 6.8 % ) were diagnosed with DIC .
	manualset3
120429	1	404046	13	NULL	NULL	0	NULL	proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of these proteins , only F-actin was identified in the apical processes of RPE cells .
	manualset3
120430	2	404046	13	NULL	NULL	0	NULL	F-actin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Of these proteins , only F-actin was identified in the apical processes of RPE cells .
	manualset3
120431	3	404046	13	NULL	NULL	0	NULL	apical processes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Of these proteins , only F-actin was identified in the apical processes of RPE cells .
	manualset3
120432	4	404046	13	NULL	NULL	0	NULL	RPE cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Of these proteins , only F-actin was identified in the apical processes of RPE cells .
	manualset3
120433	1	404047	13	NULL	NULL	0	NULL	postmicturition dribble	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of those who had experienced postmicturition dribble ; 14.0 % dribbled almost daily but the degree of postmicturition dribble was limited to spotting or wetting of the underwear in 93.2 % .
	manualset3
120434	2	404047	13	NULL	NULL	0	NULL	14.0 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of those who had experienced postmicturition dribble ; 14.0 % dribbled almost daily but the degree of postmicturition dribble was limited to spotting or wetting of the underwear in 93.2 % .
	manualset3
120435	3	404047	13	NULL	NULL	0	NULL	degree	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of those who had experienced postmicturition dribble ; 14.0 % dribbled almost daily but the degree of postmicturition dribble was limited to spotting or wetting of the underwear in 93.2 % .
	manualset3
120436	4	404047	13	NULL	NULL	0	NULL	postmicturition dribble	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of those who had experienced postmicturition dribble ; 14.0 % dribbled almost daily but the degree of postmicturition dribble was limited to spotting or wetting of the underwear in 93.2 % .
	manualset3
120437	5	404047	13	NULL	NULL	0	NULL	underwear	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Of those who had experienced postmicturition dribble ; 14.0 % dribbled almost daily but the degree of postmicturition dribble was limited to spotting or wetting of the underwear in 93.2 % .
	manualset3
120438	6	404047	13	NULL	NULL	0	NULL	93.2 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of those who had experienced postmicturition dribble ; 14.0 % dribbled almost daily but the degree of postmicturition dribble was limited to spotting or wetting of the underwear in 93.2 % .
	manualset3
120439	1	404048	13	NULL	NULL	0	NULL	country	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Of those with country of birth reported , 2598 ( 73 % ) were born in the UK and 973 ( 27 % ) abroad .
	manualset3
120440	2	404048	13	NULL	NULL	0	NULL	birth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of those with country of birth reported , 2598 ( 73 % ) were born in the UK and 973 ( 27 % ) abroad .
	manualset3
120441	3	404048	13	NULL	NULL	0	NULL	2598 ( 73 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of those with country of birth reported , 2598 ( 73 % ) were born in the UK and 973 ( 27 % ) abroad .
	manualset3
120442	4	404048	13	NULL	NULL	0	NULL	UK	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Of those with country of birth reported , 2598 ( 73 % ) were born in the UK and 973 ( 27 % ) abroad .
	manualset3
120443	5	404048	13	NULL	NULL	0	NULL	973 ( 27 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of those with country of birth reported , 2598 ( 73 % ) were born in the UK and 973 ( 27 % ) abroad .
	manualset3
120444	1	404049	13	NULL	NULL	0	NULL	uses	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Off-label uses for selective serotonin reuptake inhibitors .
	manualset3
120445	2	404049	13	NULL	NULL	0	NULL	serotonin reuptake inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Off-label uses for selective serotonin reuptake inhibitors .
	manualset3
120448	1	404050	13	NULL	NULL	0	NULL	diets 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Offered diets contained 10.2 , 14.2 , 18.3 , and 23.6 % CP ( DM basis ) , and CP concentration in consumed DM was 9.3 , 13.8 , 17.1 , and 22.1 % ( P1 , P2 , P3 , and P4 , respectively ) ; supplemental protein was from soybean meal for P1 and P2 and from soybean meal plus a blend of blood , fish , and feather meals for P3 and P4 .
	manualset3
120449	2	404050	13	NULL	NULL	0	NULL	10.2 % CP	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Offered diets contained 10.2 , 14.2 , 18.3 , and 23.6 % CP ( DM basis ) , and CP concentration in consumed DM was 9.3 , 13.8 , 17.1 , and 22.1 % ( P1 , P2 , P3 , and P4 , respectively ) ; supplemental protein was from soybean meal for P1 and P2 and from soybean meal plus a blend of blood , fish , and feather meals for P3 and P4 .
	manualset3
120450	3	404050	13	NULL	NULL	0	NULL	14.2 % CP	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Offered diets contained 10.2 , 14.2 , 18.3 , and 23.6 % CP ( DM basis ) , and CP concentration in consumed DM was 9.3 , 13.8 , 17.1 , and 22.1 % ( P1 , P2 , P3 , and P4 , respectively ) ; supplemental protein was from soybean meal for P1 and P2 and from soybean meal plus a blend of blood , fish , and feather meals for P3 and P4 .
	manualset3
120451	4	404050	13	NULL	NULL	0	NULL	18.3 % CP	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Offered diets contained 10.2 , 14.2 , 18.3 , and 23.6 % CP ( DM basis ) , and CP concentration in consumed DM was 9.3 , 13.8 , 17.1 , and 22.1 % ( P1 , P2 , P3 , and P4 , respectively ) ; supplemental protein was from soybean meal for P1 and P2 and from soybean meal plus a blend of blood , fish , and feather meals for P3 and P4 .
	manualset3
120452	5	404050	13	NULL	NULL	0	NULL	23.6 % CP	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Offered diets contained 10.2 , 14.2 , 18.3 , and 23.6 % CP ( DM basis ) , and CP concentration in consumed DM was 9.3 , 13.8 , 17.1 , and 22.1 % ( P1 , P2 , P3 , and P4 , respectively ) ; supplemental protein was from soybean meal for P1 and P2 and from soybean meal plus a blend of blood , fish , and feather meals for P3 and P4 .
	manualset3
120453	6	404050	13	NULL	NULL	0	NULL	DM basis	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Offered diets contained 10.2 , 14.2 , 18.3 , and 23.6 % CP ( DM basis ) , and CP concentration in consumed DM was 9.3 , 13.8 , 17.1 , and 22.1 % ( P1 , P2 , P3 , and P4 , respectively ) ; supplemental protein was from soybean meal for P1 and P2 and from soybean meal plus a blend of blood , fish , and feather meals for P3 and P4 .
	manualset3
120454	7	404050	13	NULL	NULL	0	NULL	CP concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Offered diets contained 10.2 , 14.2 , 18.3 , and 23.6 % CP ( DM basis ) , and CP concentration in consumed DM was 9.3 , 13.8 , 17.1 , and 22.1 % ( P1 , P2 , P3 , and P4 , respectively ) ; supplemental protein was from soybean meal for P1 and P2 and from soybean meal plus a blend of blood , fish , and feather meals for P3 and P4 .
	manualset3
120455	8	404050	13	NULL	NULL	0	NULL	DM 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Offered diets contained 10.2 , 14.2 , 18.3 , and 23.6 % CP ( DM basis ) , and CP concentration in consumed DM was 9.3 , 13.8 , 17.1 , and 22.1 % ( P1 , P2 , P3 , and P4 , respectively ) ; supplemental protein was from soybean meal for P1 and P2 and from soybean meal plus a blend of blood , fish , and feather meals for P3 and P4 .
	manualset3
120456	9	404050	13	NULL	NULL	0	NULL	9.3 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Offered diets contained 10.2 , 14.2 , 18.3 , and 23.6 % CP ( DM basis ) , and CP concentration in consumed DM was 9.3 , 13.8 , 17.1 , and 22.1 % ( P1 , P2 , P3 , and P4 , respectively ) ; supplemental protein was from soybean meal for P1 and P2 and from soybean meal plus a blend of blood , fish , and feather meals for P3 and P4 .
	manualset3
120457	10	404050	13	NULL	NULL	0	NULL	13.8 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Offered diets contained 10.2 , 14.2 , 18.3 , and 23.6 % CP ( DM basis ) , and CP concentration in consumed DM was 9.3 , 13.8 , 17.1 , and 22.1 % ( P1 , P2 , P3 , and P4 , respectively ) ; supplemental protein was from soybean meal for P1 and P2 and from soybean meal plus a blend of blood , fish , and feather meals for P3 and P4 .
	manualset3
120458	11	404050	13	NULL	NULL	0	NULL	17.1%	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Offered diets contained 10.2 , 14.2 , 18.3 , and 23.6 % CP ( DM basis ) , and CP concentration in consumed DM was 9.3 , 13.8 , 17.1 , and 22.1 % ( P1 , P2 , P3 , and P4 , respectively ) ; supplemental protein was from soybean meal for P1 and P2 and from soybean meal plus a blend of blood , fish , and feather meals for P3 and P4 .
	manualset3
120459	12	404050	13	NULL	NULL	0	NULL	22.1 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Offered diets contained 10.2 , 14.2 , 18.3 , and 23.6 % CP ( DM basis ) , and CP concentration in consumed DM was 9.3 , 13.8 , 17.1 , and 22.1 % ( P1 , P2 , P3 , and P4 , respectively ) ; supplemental protein was from soybean meal for P1 and P2 and from soybean meal plus a blend of blood , fish , and feather meals for P3 and P4 .
	manualset3
120460	13	404050	13	NULL	NULL	NULL	NULL	P1	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Offered diets contained 10.2 , 14.2 , 18.3 , and 23.6 % CP ( DM basis ) , and CP concentration in consumed DM was 9.3 , 13.8 , 17.1 , and 22.1 % ( P1 , P2 , P3 , and P4 , respectively ) ; supplemental protein was from soybean meal for P1 and P2 and from soybean meal plus a blend of blood , fish , and feather meals for P3 and P4 .
	manualset3
120461	14	404050	13	NULL	NULL	NULL	NULL	P2	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Offered diets contained 10.2 , 14.2 , 18.3 , and 23.6 % CP ( DM basis ) , and CP concentration in consumed DM was 9.3 , 13.8 , 17.1 , and 22.1 % ( P1 , P2 , P3 , and P4 , respectively ) ; supplemental protein was from soybean meal for P1 and P2 and from soybean meal plus a blend of blood , fish , and feather meals for P3 and P4 .
	manualset3
120462	15	404050	13	NULL	NULL	NULL	NULL	P3	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Offered diets contained 10.2 , 14.2 , 18.3 , and 23.6 % CP ( DM basis ) , and CP concentration in consumed DM was 9.3 , 13.8 , 17.1 , and 22.1 % ( P1 , P2 , P3 , and P4 , respectively ) ; supplemental protein was from soybean meal for P1 and P2 and from soybean meal plus a blend of blood , fish , and feather meals for P3 and P4 .
	manualset3
120463	16	404050	13	NULL	NULL	NULL	NULL	P4 	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Offered diets contained 10.2 , 14.2 , 18.3 , and 23.6 % CP ( DM basis ) , and CP concentration in consumed DM was 9.3 , 13.8 , 17.1 , and 22.1 % ( P1 , P2 , P3 , and P4 , respectively ) ; supplemental protein was from soybean meal for P1 and P2 and from soybean meal plus a blend of blood , fish , and feather meals for P3 and P4 .
	manualset3
120464	17	404050	13	NULL	NULL	0	NULL	supplemental protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Offered diets contained 10.2 , 14.2 , 18.3 , and 23.6 % CP ( DM basis ) , and CP concentration in consumed DM was 9.3 , 13.8 , 17.1 , and 22.1 % ( P1 , P2 , P3 , and P4 , respectively ) ; supplemental protein was from soybean meal for P1 and P2 and from soybean meal plus a blend of blood , fish , and feather meals for P3 and P4 .
	manualset3
120465	18	404050	13	NULL	NULL	0	NULL	soybean meal	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Offered diets contained 10.2 , 14.2 , 18.3 , and 23.6 % CP ( DM basis ) , and CP concentration in consumed DM was 9.3 , 13.8 , 17.1 , and 22.1 % ( P1 , P2 , P3 , and P4 , respectively ) ; supplemental protein was from soybean meal for P1 and P2 and from soybean meal plus a blend of blood , fish , and feather meals for P3 and P4 .
	manualset3
120466	19	404050	13	NULL	NULL	0	NULL	P1	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Offered diets contained 10.2 , 14.2 , 18.3 , and 23.6 % CP ( DM basis ) , and CP concentration in consumed DM was 9.3 , 13.8 , 17.1 , and 22.1 % ( P1 , P2 , P3 , and P4 , respectively ) ; supplemental protein was from soybean meal for P1 and P2 and from soybean meal plus a blend of blood , fish , and feather meals for P3 and P4 .
	manualset3
120467	20	404050	13	NULL	NULL	0	NULL	P2	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Offered diets contained 10.2 , 14.2 , 18.3 , and 23.6 % CP ( DM basis ) , and CP concentration in consumed DM was 9.3 , 13.8 , 17.1 , and 22.1 % ( P1 , P2 , P3 , and P4 , respectively ) ; supplemental protein was from soybean meal for P1 and P2 and from soybean meal plus a blend of blood , fish , and feather meals for P3 and P4 .
	manualset3
120468	21	404050	13	NULL	NULL	0	NULL	soybean meal	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Offered diets contained 10.2 , 14.2 , 18.3 , and 23.6 % CP ( DM basis ) , and CP concentration in consumed DM was 9.3 , 13.8 , 17.1 , and 22.1 % ( P1 , P2 , P3 , and P4 , respectively ) ; supplemental protein was from soybean meal for P1 and P2 and from soybean meal plus a blend of blood , fish , and feather meals for P3 and P4 .
	manualset3
120469	22	404050	13	NULL	NULL	0	NULL	blend	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Offered diets contained 10.2 , 14.2 , 18.3 , and 23.6 % CP ( DM basis ) , and CP concentration in consumed DM was 9.3 , 13.8 , 17.1 , and 22.1 % ( P1 , P2 , P3 , and P4 , respectively ) ; supplemental protein was from soybean meal for P1 and P2 and from soybean meal plus a blend of blood , fish , and feather meals for P3 and P4 .
	manualset3
120470	23	404050	13	NULL	NULL	0	NULL	blood meals	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Offered diets contained 10.2 , 14.2 , 18.3 , and 23.6 % CP ( DM basis ) , and CP concentration in consumed DM was 9.3 , 13.8 , 17.1 , and 22.1 % ( P1 , P2 , P3 , and P4 , respectively ) ; supplemental protein was from soybean meal for P1 and P2 and from soybean meal plus a blend of blood , fish , and feather meals for P3 and P4 .
	manualset3
120471	24	404050	13	NULL	NULL	0	NULL	fish meals	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Offered diets contained 10.2 , 14.2 , 18.3 , and 23.6 % CP ( DM basis ) , and CP concentration in consumed DM was 9.3 , 13.8 , 17.1 , and 22.1 % ( P1 , P2 , P3 , and P4 , respectively ) ; supplemental protein was from soybean meal for P1 and P2 and from soybean meal plus a blend of blood , fish , and feather meals for P3 and P4 .
	manualset3
120472	25	404050	13	NULL	NULL	0	NULL	feather meals	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Offered diets contained 10.2 , 14.2 , 18.3 , and 23.6 % CP ( DM basis ) , and CP concentration in consumed DM was 9.3 , 13.8 , 17.1 , and 22.1 % ( P1 , P2 , P3 , and P4 , respectively ) ; supplemental protein was from soybean meal for P1 and P2 and from soybean meal plus a blend of blood , fish , and feather meals for P3 and P4 .
	manualset3
120473	26	404050	13	NULL	NULL	0	NULL	P3	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Offered diets contained 10.2 , 14.2 , 18.3 , and 23.6 % CP ( DM basis ) , and CP concentration in consumed DM was 9.3 , 13.8 , 17.1 , and 22.1 % ( P1 , P2 , P3 , and P4 , respectively ) ; supplemental protein was from soybean meal for P1 and P2 and from soybean meal plus a blend of blood , fish , and feather meals for P3 and P4 .
	manualset3
120474	27	404050	13	NULL	NULL	0	NULL	P4 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Offered diets contained 10.2 , 14.2 , 18.3 , and 23.6 % CP ( DM basis ) , and CP concentration in consumed DM was 9.3 , 13.8 , 17.1 , and 22.1 % ( P1 , P2 , P3 , and P4 , respectively ) ; supplemental protein was from soybean meal for P1 and P2 and from soybean meal plus a blend of blood , fish , and feather meals for P3 and P4 .
	manualset3
120475	1	404051	13	NULL	NULL	0	NULL	decisive place	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A decisive place in the prevention of VHC transmission in dialyzed subjects is held by non-specific preventive measures , transfusions are most probably not the decisive vehicle .
	manualset3
120476	2	404051	13	NULL	NULL	0	NULL	prevention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A decisive place in the prevention of VHC transmission in dialyzed subjects is held by non-specific preventive measures , transfusions are most probably not the decisive vehicle .
	manualset3
120477	3	404051	13	NULL	NULL	0	NULL	VHC transmission	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A decisive place in the prevention of VHC transmission in dialyzed subjects is held by non-specific preventive measures , transfusions are most probably not the decisive vehicle .
	manualset3
120478	4	404051	13	NULL	NULL	0	NULL	dialyzed subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A decisive place in the prevention of VHC transmission in dialyzed subjects is held by non-specific preventive measures , transfusions are most probably not the decisive vehicle .
	manualset3
120479	5	404051	13	NULL	NULL	0	NULL	preventive measures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A decisive place in the prevention of VHC transmission in dialyzed subjects is held by non-specific preventive measures , transfusions are most probably not the decisive vehicle .
	manualset3
120480	6	404051	13	NULL	NULL	0	NULL	transfusions 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A decisive place in the prevention of VHC transmission in dialyzed subjects is held by non-specific preventive measures , transfusions are most probably not the decisive vehicle .
	manualset3
120481	7	404051	13	NULL	NULL	0	NULL	decisive vehicle	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A decisive place in the prevention of VHC transmission in dialyzed subjects is held by non-specific preventive measures , transfusions are most probably not the decisive vehicle .
	manualset3
120482	1	404052	13	NULL	NULL	0	NULL	Offspring 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Offspring of mother mice treated immediately after delivery with deaggregated human gamma-globulins ( dHGG ) are unable to produce HGG-specific antibodies when challenged with immunogenic forms of HGG ( HGG/CFA ) in adulthood .
	manualset3
120483	2	404052	13	NULL	NULL	0	NULL	mother mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Offspring of mother mice treated immediately after delivery with deaggregated human gamma-globulins ( dHGG ) are unable to produce HGG-specific antibodies when challenged with immunogenic forms of HGG ( HGG/CFA ) in adulthood .
	manualset3
120484	3	404052	13	NULL	NULL	0	NULL	delivery	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Offspring of mother mice treated immediately after delivery with deaggregated human gamma-globulins ( dHGG ) are unable to produce HGG-specific antibodies when challenged with immunogenic forms of HGG ( HGG/CFA ) in adulthood .
	manualset3
120485	4	404052	13	NULL	NULL	0	NULL	deaggregated human gamma-globulins ( dHGG )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Offspring of mother mice treated immediately after delivery with deaggregated human gamma-globulins ( dHGG ) are unable to produce HGG-specific antibodies when challenged with immunogenic forms of HGG ( HGG/CFA ) in adulthood .
	manualset3
120486	5	404052	13	NULL	NULL	0	NULL	HGG-specific antibodies 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Offspring of mother mice treated immediately after delivery with deaggregated human gamma-globulins ( dHGG ) are unable to produce HGG-specific antibodies when challenged with immunogenic forms of HGG ( HGG/CFA ) in adulthood .
	manualset3
120487	6	404052	13	NULL	NULL	0	NULL	immunogenic forms of HGG ( HGG/CFA )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Offspring of mother mice treated immediately after delivery with deaggregated human gamma-globulins ( dHGG ) are unable to produce HGG-specific antibodies when challenged with immunogenic forms of HGG ( HGG/CFA ) in adulthood .
	manualset3
120488	7	404052	13	NULL	NULL	0	NULL	adulthood	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Offspring of mother mice treated immediately after delivery with deaggregated human gamma-globulins ( dHGG ) are unable to produce HGG-specific antibodies when challenged with immunogenic forms of HGG ( HGG/CFA ) in adulthood .
	manualset3
120489	1	404053	13	NULL	NULL	0	NULL	condition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Often misdiagnosed as a condition simply of weight loss , cachexia is actually a highly complex metabolic disorder involving features of anorexia , anemia , lipolysis and insulin resistance .
	manualset3
120490	2	404053	13	NULL	NULL	0	NULL	weight loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Often misdiagnosed as a condition simply of weight loss , cachexia is actually a highly complex metabolic disorder involving features of anorexia , anemia , lipolysis and insulin resistance .
	manualset3
120491	3	404053	13	NULL	NULL	0	NULL	cachexia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Often misdiagnosed as a condition simply of weight loss , cachexia is actually a highly complex metabolic disorder involving features of anorexia , anemia , lipolysis and insulin resistance .
	manualset3
120492	4	404053	13	NULL	NULL	0	NULL	complex metabolic disorder	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Often misdiagnosed as a condition simply of weight loss , cachexia is actually a highly complex metabolic disorder involving features of anorexia , anemia , lipolysis and insulin resistance .
	manualset3
120493	5	404053	13	NULL	NULL	0	NULL	features	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Often misdiagnosed as a condition simply of weight loss , cachexia is actually a highly complex metabolic disorder involving features of anorexia , anemia , lipolysis and insulin resistance .
	manualset3
120494	6	404053	13	NULL	NULL	0	NULL	anorexia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Often misdiagnosed as a condition simply of weight loss , cachexia is actually a highly complex metabolic disorder involving features of anorexia , anemia , lipolysis and insulin resistance .
	manualset3
120495	7	404053	13	NULL	NULL	0	NULL	anemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Often misdiagnosed as a condition simply of weight loss , cachexia is actually a highly complex metabolic disorder involving features of anorexia , anemia , lipolysis and insulin resistance .
	manualset3
120496	8	404053	13	NULL	NULL	0	NULL	lipolysis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Often misdiagnosed as a condition simply of weight loss , cachexia is actually a highly complex metabolic disorder involving features of anorexia , anemia , lipolysis and insulin resistance .
	manualset3
120497	9	404053	13	NULL	NULL	0	NULL	insulin resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Often misdiagnosed as a condition simply of weight loss , cachexia is actually a highly complex metabolic disorder involving features of anorexia , anemia , lipolysis and insulin resistance .
	manualset3
120968	1	404054	13	NULL	NULL	0	NULL	Old female rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Old female rats ( 20-27 months ) were given acute administration of an indirectly acting dopamine ( DA ) agonist , nomifensine or scalar doses of the direct DA receptor agonist , bromocriptine .
	manualset3
120969	2	404054	13	NULL	NULL	0	NULL	20-27 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Old female rats ( 20-27 months ) were given acute administration of an indirectly acting dopamine ( DA ) agonist , nomifensine or scalar doses of the direct DA receptor agonist , bromocriptine .
	manualset3
120970	3	404054	13	NULL	NULL	0	NULL	acute administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Old female rats ( 20-27 months ) were given acute administration of an indirectly acting dopamine ( DA ) agonist , nomifensine or scalar doses of the direct DA receptor agonist , bromocriptine .
	manualset3
120971	4	404054	13	NULL	NULL	NULL	NULL	dopamine ( DA ) agonist	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Old female rats ( 20-27 months ) were given acute administration of an indirectly acting dopamine ( DA ) agonist , nomifensine or scalar doses of the direct DA receptor agonist , bromocriptine .
	manualset3
120972	5	404054	13	NULL	NULL	0	NULL	 nomifensine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Old female rats ( 20-27 months ) were given acute administration of an indirectly acting dopamine ( DA ) agonist , nomifensine or scalar doses of the direct DA receptor agonist , bromocriptine .
	manualset3
120973	6	404054	13	NULL	NULL	0	NULL	scalar doses 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Old female rats ( 20-27 months ) were given acute administration of an indirectly acting dopamine ( DA ) agonist , nomifensine or scalar doses of the direct DA receptor agonist , bromocriptine .
	manualset3
120974	7	404054	13	NULL	NULL	0	NULL	DA receptor agonist	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Old female rats ( 20-27 months ) were given acute administration of an indirectly acting dopamine ( DA ) agonist , nomifensine or scalar doses of the direct DA receptor agonist , bromocriptine .
	manualset3
120975	8	404054	13	NULL	NULL	0	NULL	bromocriptine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Old female rats ( 20-27 months ) were given acute administration of an indirectly acting dopamine ( DA ) agonist , nomifensine or scalar doses of the direct DA receptor agonist , bromocriptine .
	manualset3
120976	1	404055	13	NULL	NULL	0	NULL	Old world tree	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Old world tree found in Colombia .
	manualset3
120977	2	404055	13	NULL	NULL	0	NULL	Colombia 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Old world tree found in Colombia .
	manualset3
120978	1	404056	13	NULL	NULL	0	NULL	Older NLS patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Older NLS patients were likely to have a diagnosis of schizophrenia ( 79.6 % ) , followed by mood disorder ( 6.1 % ) and dementia ( 4.1 % ) .
	manualset3
120979	2	404056	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Older NLS patients were likely to have a diagnosis of schizophrenia ( 79.6 % ) , followed by mood disorder ( 6.1 % ) and dementia ( 4.1 % ) .
	manualset3
120980	3	404056	13	NULL	NULL	0	NULL	schizophrenia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Older NLS patients were likely to have a diagnosis of schizophrenia ( 79.6 % ) , followed by mood disorder ( 6.1 % ) and dementia ( 4.1 % ) .
	manualset3
120981	4	404056	13	NULL	NULL	0	NULL	79.6 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Older NLS patients were likely to have a diagnosis of schizophrenia ( 79.6 % ) , followed by mood disorder ( 6.1 % ) and dementia ( 4.1 % ) .
	manualset3
120982	5	404056	13	NULL	NULL	NULL	NULL	mood disorder	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Older NLS patients were likely to have a diagnosis of schizophrenia ( 79.6 % ) , followed by mood disorder ( 6.1 % ) and dementia ( 4.1 % ) .
	manualset3
120983	6	404056	13	NULL	NULL	0	NULL	6.1 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Older NLS patients were likely to have a diagnosis of schizophrenia ( 79.6 % ) , followed by mood disorder ( 6.1 % ) and dementia ( 4.1 % ) .
	manualset3
120984	7	404056	13	NULL	NULL	0	NULL	dementia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Older NLS patients were likely to have a diagnosis of schizophrenia ( 79.6 % ) , followed by mood disorder ( 6.1 % ) and dementia ( 4.1 % ) .
	manualset3
120985	8	404056	13	NULL	NULL	0	NULL	4.1 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Older NLS patients were likely to have a diagnosis of schizophrenia ( 79.6 % ) , followed by mood disorder ( 6.1 % ) and dementia ( 4.1 % ) .
	manualset3
120986	1	404057	13	NULL	NULL	0	NULL	Older adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Older adults who have chronic diseases or chronic infections are more susceptible to common infections and have poor vaccine responses .
	manualset3
120987	2	404057	13	NULL	NULL	0	NULL	chronic diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Older adults who have chronic diseases or chronic infections are more susceptible to common infections and have poor vaccine responses .
	manualset3
120988	3	404057	13	NULL	NULL	0	NULL	chronic infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Older adults who have chronic diseases or chronic infections are more susceptible to common infections and have poor vaccine responses .
	manualset3
120989	4	404057	13	NULL	NULL	NULL	NULL	common infections 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Older adults who have chronic diseases or chronic infections are more susceptible to common infections and have poor vaccine responses .
	manualset3
120990	5	404057	13	NULL	NULL	0	NULL	poor vaccine responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Older adults who have chronic diseases or chronic infections are more susceptible to common infections and have poor vaccine responses .
	manualset3
120991	1	404058	13	NULL	NULL	0	NULL	Oleic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Oleic acid was the main unsaturated fatty acid found in the tumor tissue .
	manualset3
120992	2	404058	13	NULL	NULL	0	NULL	unsaturated fatty acid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Oleic acid was the main unsaturated fatty acid found in the tumor tissue .
	manualset3
120993	3	404058	13	NULL	NULL	0	NULL	tumor tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Oleic acid was the main unsaturated fatty acid found in the tumor tissue .
	manualset3
120994	1	404059	13	NULL	NULL	0	NULL	Oligogenic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Oligogenic analysis accounting simultaneously for the contribution of this locus on chromosome 18 and other chromosomal regions showing some evidence of linkage in these Caucasian families ( on chromosomes 2 , 4 and 20 ) failed to yield significant evidence for interaction .
	manualset3
120996	3	404059	13	NULL	NULL	0	NULL	contribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Oligogenic analysis accounting simultaneously for the contribution of this locus on chromosome 18 and other chromosomal regions showing some evidence of linkage in these Caucasian families ( on chromosomes 2 , 4 and 20 ) failed to yield significant evidence for interaction .
	manualset3
120997	4	404059	13	NULL	NULL	0	NULL	locus on chromosome 18	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Oligogenic analysis accounting simultaneously for the contribution of this locus on chromosome 18 and other chromosomal regions showing some evidence of linkage in these Caucasian families ( on chromosomes 2 , 4 and 20 ) failed to yield significant evidence for interaction .
	manualset3
120998	5	404059	13	NULL	NULL	0	NULL	chromosomal regions	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Oligogenic analysis accounting simultaneously for the contribution of this locus on chromosome 18 and other chromosomal regions showing some evidence of linkage in these Caucasian families ( on chromosomes 2 , 4 and 20 ) failed to yield significant evidence for interaction .
	manualset3
120999	6	404059	13	NULL	NULL	NULL	NULL	evidence	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Oligogenic analysis accounting simultaneously for the contribution of this locus on chromosome 18 and other chromosomal regions showing some evidence of linkage in these Caucasian families ( on chromosomes 2 , 4 and 20 ) failed to yield significant evidence for interaction .
	manualset3
121000	7	404059	13	NULL	NULL	0	NULL	linkage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Oligogenic analysis accounting simultaneously for the contribution of this locus on chromosome 18 and other chromosomal regions showing some evidence of linkage in these Caucasian families ( on chromosomes 2 , 4 and 20 ) failed to yield significant evidence for interaction .
	manualset3
121001	8	404059	13	NULL	NULL	0	NULL	Caucasian families	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Oligogenic analysis accounting simultaneously for the contribution of this locus on chromosome 18 and other chromosomal regions showing some evidence of linkage in these Caucasian families ( on chromosomes 2 , 4 and 20 ) failed to yield significant evidence for interaction .
	manualset3
121002	9	404059	13	NULL	NULL	0	NULL	chromosome 2	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Oligogenic analysis accounting simultaneously for the contribution of this locus on chromosome 18 and other chromosomal regions showing some evidence of linkage in these Caucasian families ( on chromosomes 2 , 4 and 20 ) failed to yield significant evidence for interaction .
	manualset3
121003	10	404059	13	NULL	NULL	0	NULL	chromosome 4	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Oligogenic analysis accounting simultaneously for the contribution of this locus on chromosome 18 and other chromosomal regions showing some evidence of linkage in these Caucasian families ( on chromosomes 2 , 4 and 20 ) failed to yield significant evidence for interaction .
	manualset3
121004	11	404059	13	NULL	NULL	0	NULL	chromosome 20	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Oligogenic analysis accounting simultaneously for the contribution of this locus on chromosome 18 and other chromosomal regions showing some evidence of linkage in these Caucasian families ( on chromosomes 2 , 4 and 20 ) failed to yield significant evidence for interaction .
	manualset3
121005	12	404059	13	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Oligogenic analysis accounting simultaneously for the contribution of this locus on chromosome 18 and other chromosomal regions showing some evidence of linkage in these Caucasian families ( on chromosomes 2 , 4 and 20 ) failed to yield significant evidence for interaction .
	manualset3
121006	13	404059	13	NULL	NULL	0	NULL	interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Oligogenic analysis accounting simultaneously for the contribution of this locus on chromosome 18 and other chromosomal regions showing some evidence of linkage in these Caucasian families ( on chromosomes 2 , 4 and 20 ) failed to yield significant evidence for interaction .
	manualset3
121007	1	404060	13	NULL	NULL	0	NULL	Oligomerization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Oligomerization of NHERF-1 and NHERF-2 PDZ domains : differential regulation by association with receptor carboxyl-termini and by phosphorylation .
	manualset3
121008	2	404060	13	NULL	NULL	0	NULL	NHERF-1 PDZ domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Oligomerization of NHERF-1 and NHERF-2 PDZ domains : differential regulation by association with receptor carboxyl-termini and by phosphorylation .
	manualset3
121009	3	404060	13	NULL	NULL	0	NULL	 NHERF-2 PDZ domains 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Oligomerization of NHERF-1 and NHERF-2 PDZ domains : differential regulation by association with receptor carboxyl-termini and by phosphorylation .
	manualset3
121010	4	404060	13	NULL	NULL	0	NULL	regulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Oligomerization of NHERF-1 and NHERF-2 PDZ domains : differential regulation by association with receptor carboxyl-termini and by phosphorylation .
	manualset3
121011	5	404060	13	NULL	NULL	0	NULL	association 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Oligomerization of NHERF-1 and NHERF-2 PDZ domains : differential regulation by association with receptor carboxyl-termini and by phosphorylation .
	manualset3
121012	6	404060	13	NULL	NULL	0	NULL	 receptor carboxyl-termini	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Oligomerization of NHERF-1 and NHERF-2 PDZ domains : differential regulation by association with receptor carboxyl-termini and by phosphorylation .
	manualset3
121013	7	404060	13	NULL	NULL	0	NULL	phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Oligomerization of NHERF-1 and NHERF-2 PDZ domains : differential regulation by association with receptor carboxyl-termini and by phosphorylation .
	manualset3
121014	1	404061	13	NULL	NULL	0	NULL	Oligonucleotide primers 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Oligonucleotide primers were constructed that corresponded to the above-mentioned amino acid sequences and polymerase chain reactions were performed in zebrafish ( Brachydanio rerio ) and masu salmon ( Oncorynchus masou ) embryos .
	manualset3
121015	2	404061	13	NULL	NULL	0	NULL	amino acid sequences	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Oligonucleotide primers were constructed that corresponded to the above-mentioned amino acid sequences and polymerase chain reactions were performed in zebrafish ( Brachydanio rerio ) and masu salmon ( Oncorynchus masou ) embryos .
	manualset3
121016	3	404061	13	NULL	NULL	0	NULL	polymerase chain reactions	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Oligonucleotide primers were constructed that corresponded to the above-mentioned amino acid sequences and polymerase chain reactions were performed in zebrafish ( Brachydanio rerio ) and masu salmon ( Oncorynchus masou ) embryos .
	manualset3
121017	4	404061	13	NULL	NULL	0	NULL	zebrafish ( Brachydanio rerio ) embryos	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Oligonucleotide primers were constructed that corresponded to the above-mentioned amino acid sequences and polymerase chain reactions were performed in zebrafish ( Brachydanio rerio ) and masu salmon ( Oncorynchus masou ) embryos .
	manualset3
121018	5	404061	13	NULL	NULL	0	NULL	masu salmon ( Oncorynchus masou ) embryos 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Oligonucleotide primers were constructed that corresponded to the above-mentioned amino acid sequences and polymerase chain reactions were performed in zebrafish ( Brachydanio rerio ) and masu salmon ( Oncorynchus masou ) embryos .
	manualset3
121019	1	404062	13	NULL	NULL	0	NULL	Omission	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Omission of penicillin from the medium resulted in development of short bacterial forms .
	manualset3
121020	2	404062	13	NULL	NULL	0	NULL	penicillin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Omission of penicillin from the medium resulted in development of short bacterial forms .
	manualset3
121021	3	404062	13	NULL	NULL	0	NULL	medium	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Omission of penicillin from the medium resulted in development of short bacterial forms .
	manualset3
121022	4	404062	13	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Omission of penicillin from the medium resulted in development of short bacterial forms .
	manualset3
121023	5	404062	13	NULL	NULL	0	NULL	short bacterial forms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Omission of penicillin from the medium resulted in development of short bacterial forms .
	manualset3
121024	1	404063	13	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Omitting the use of nitrous oxide even renders it possible to perform closed-system anaesthesia with conventional anesthetic machines in routine clinical practice .
	manualset3
121025	2	404063	13	NULL	NULL	0	NULL	nitrous oxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Omitting the use of nitrous oxide even renders it possible to perform closed-system anaesthesia with conventional anesthetic machines in routine clinical practice .
	manualset3
121026	3	404063	13	NULL	NULL	0	NULL	closed-system anaesthesia 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Omitting the use of nitrous oxide even renders it possible to perform closed-system anaesthesia with conventional anesthetic machines in routine clinical practice .
	manualset3
121027	4	404063	13	NULL	NULL	0	NULL	conventional anesthetic machines	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Omitting the use of nitrous oxide even renders it possible to perform closed-system anaesthesia with conventional anesthetic machines in routine clinical practice .
	manualset3
121028	5	404063	13	NULL	NULL	0	NULL	routine clinical practice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Omitting the use of nitrous oxide even renders it possible to perform closed-system anaesthesia with conventional anesthetic machines in routine clinical practice .
	manualset3
120995	4	404064	13	NULL	NULL	NULL	NULL	absentee	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On-call supervision and resident autonomy : from micromanager to absentee attending .
	manualset3
121029	1	404064	13	NULL	NULL	0	NULL	On-call supervision 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	On-call supervision and resident autonomy : from micromanager to absentee attending .
	manualset3
121030	2	404064	13	NULL	NULL	0	NULL	resident autonomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	On-call supervision and resident autonomy : from micromanager to absentee attending .
	manualset3
121031	3	404064	13	NULL	NULL	0	NULL	micromanager	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	On-call supervision and resident autonomy : from micromanager to absentee attending .
	manualset3
121032	1	404065	13	NULL	NULL	0	NULL	requirements	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On-demand requirements of patients with endoscopy-negative gastro-oesophageal reflux disease : H2-blocker vs. proton pump inhibitor .
	manualset3
121033	2	404065	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On-demand requirements of patients with endoscopy-negative gastro-oesophageal reflux disease : H2-blocker vs. proton pump inhibitor .
	manualset3
121034	3	404065	13	NULL	NULL	0	NULL	endoscopy-negative gastro-oesophageal reflux disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	On-demand requirements of patients with endoscopy-negative gastro-oesophageal reflux disease : H2-blocker vs. proton pump inhibitor .
	manualset3
121035	4	404065	13	NULL	NULL	0	NULL	H2-blocker	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On-demand requirements of patients with endoscopy-negative gastro-oesophageal reflux disease : H2-blocker vs. proton pump inhibitor .
	manualset3
121036	5	404065	13	NULL	NULL	0	NULL	proton pump inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On-demand requirements of patients with endoscopy-negative gastro-oesophageal reflux disease : H2-blocker vs. proton pump inhibitor .
	manualset3
121037	1	404066	13	NULL	NULL	0	NULL	decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A decrease in promoter methylation , and increase in expression of the melanocyte late-differentiation driver SOX9 , was followed by increases in cyclin-dependent kinase inhibitors ( CDKN ) p27/CDKN1B and p21/CDKN1A that mediate cell cycle exit with differentiation .
	manualset3
121038	2	404066	13	NULL	NULL	0	NULL	promoter methylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A decrease in promoter methylation , and increase in expression of the melanocyte late-differentiation driver SOX9 , was followed by increases in cyclin-dependent kinase inhibitors ( CDKN ) p27/CDKN1B and p21/CDKN1A that mediate cell cycle exit with differentiation .
	manualset3
121039	3	404066	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A decrease in promoter methylation , and increase in expression of the melanocyte late-differentiation driver SOX9 , was followed by increases in cyclin-dependent kinase inhibitors ( CDKN ) p27/CDKN1B and p21/CDKN1A that mediate cell cycle exit with differentiation .
	manualset3
121040	4	404066	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A decrease in promoter methylation , and increase in expression of the melanocyte late-differentiation driver SOX9 , was followed by increases in cyclin-dependent kinase inhibitors ( CDKN ) p27/CDKN1B and p21/CDKN1A that mediate cell cycle exit with differentiation .
	manualset3
121041	5	404066	13	NULL	NULL	0	NULL	melanocyte late-differentiation driver SOX9	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A decrease in promoter methylation , and increase in expression of the melanocyte late-differentiation driver SOX9 , was followed by increases in cyclin-dependent kinase inhibitors ( CDKN ) p27/CDKN1B and p21/CDKN1A that mediate cell cycle exit with differentiation .
	manualset3
121042	6	404066	13	NULL	NULL	0	NULL	increases	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A decrease in promoter methylation , and increase in expression of the melanocyte late-differentiation driver SOX9 , was followed by increases in cyclin-dependent kinase inhibitors ( CDKN ) p27/CDKN1B and p21/CDKN1A that mediate cell cycle exit with differentiation .
	manualset3
121043	7	404066	13	NULL	NULL	0	NULL	cyclin-dependent kinase inhibitors ( CDKN ) 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A decrease in promoter methylation , and increase in expression of the melanocyte late-differentiation driver SOX9 , was followed by increases in cyclin-dependent kinase inhibitors ( CDKN ) p27/CDKN1B and p21/CDKN1A that mediate cell cycle exit with differentiation .
	manualset3
121044	8	404066	13	NULL	NULL	0	NULL	 p27/CDKN1B 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A decrease in promoter methylation , and increase in expression of the melanocyte late-differentiation driver SOX9 , was followed by increases in cyclin-dependent kinase inhibitors ( CDKN ) p27/CDKN1B and p21/CDKN1A that mediate cell cycle exit with differentiation .
	manualset3
121045	9	404066	13	NULL	NULL	0	NULL	p21/CDKN1A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A decrease in promoter methylation , and increase in expression of the melanocyte late-differentiation driver SOX9 , was followed by increases in cyclin-dependent kinase inhibitors ( CDKN ) p27/CDKN1B and p21/CDKN1A that mediate cell cycle exit with differentiation .
	manualset3
121046	10	404066	13	NULL	NULL	0	NULL	cell cycle exit 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A decrease in promoter methylation , and increase in expression of the melanocyte late-differentiation driver SOX9 , was followed by increases in cyclin-dependent kinase inhibitors ( CDKN ) p27/CDKN1B and p21/CDKN1A that mediate cell cycle exit with differentiation .
	manualset3
121047	11	404066	13	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A decrease in promoter methylation , and increase in expression of the melanocyte late-differentiation driver SOX9 , was followed by increases in cyclin-dependent kinase inhibitors ( CDKN ) p27/CDKN1B and p21/CDKN1A that mediate cell cycle exit with differentiation .
	manualset3
121048	1	404067	13	NULL	NULL	0	NULL	On-line CI analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	On-line CI analysis was also performed with chromosomes isolated from a transitional cell carcinoma of the bladder .
	manualset3
121049	2	404067	13	NULL	NULL	0	NULL	chromosomes	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	On-line CI analysis was also performed with chromosomes isolated from a transitional cell carcinoma of the bladder .
	manualset3
121050	3	404067	13	NULL	NULL	0	NULL	transitional cell carcinoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On-line CI analysis was also performed with chromosomes isolated from a transitional cell carcinoma of the bladder .
	manualset3
121051	4	404067	13	NULL	NULL	0	NULL	bladder	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	On-line CI analysis was also performed with chromosomes isolated from a transitional cell carcinoma of the bladder .
	manualset3
121052	1	404068	13	NULL	NULL	0	NULL	April 6	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	On April 6 , 2004 , we published an interim final rule in the Federal Register implementing the provisions of the Medicare Prescription Drug , Improvement , and Modernization Act of 2003 ( MMA ) related to the calculation and submission of manufacturer 's average sales price ( ASP ) data on certain Medicare Part B drugs and biologicals by manufacturers .
	manualset3
121053	2	404068	13	NULL	NULL	0	NULL	2004	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	On April 6 , 2004 , we published an interim final rule in the Federal Register implementing the provisions of the Medicare Prescription Drug , Improvement , and Modernization Act of 2003 ( MMA ) related to the calculation and submission of manufacturer 's average sales price ( ASP ) data on certain Medicare Part B drugs and biologicals by manufacturers .
	manualset3
121054	3	404068	13	NULL	NULL	0	NULL	interim final rule	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	On April 6 , 2004 , we published an interim final rule in the Federal Register implementing the provisions of the Medicare Prescription Drug , Improvement , and Modernization Act of 2003 ( MMA ) related to the calculation and submission of manufacturer 's average sales price ( ASP ) data on certain Medicare Part B drugs and biologicals by manufacturers .
	manualset3
121055	4	404068	13	NULL	NULL	0	NULL	Federal Register 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	On April 6 , 2004 , we published an interim final rule in the Federal Register implementing the provisions of the Medicare Prescription Drug , Improvement , and Modernization Act of 2003 ( MMA ) related to the calculation and submission of manufacturer 's average sales price ( ASP ) data on certain Medicare Part B drugs and biologicals by manufacturers .
	manualset3
121056	5	404068	13	NULL	NULL	0	NULL	provisions	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	On April 6 , 2004 , we published an interim final rule in the Federal Register implementing the provisions of the Medicare Prescription Drug , Improvement , and Modernization Act of 2003 ( MMA ) related to the calculation and submission of manufacturer 's average sales price ( ASP ) data on certain Medicare Part B drugs and biologicals by manufacturers .
	manualset3
121057	6	404068	13	NULL	NULL	0	NULL	Medicare Prescription Drug , Improvement , and Modernization Act of 2003 ( MMA ) 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	On April 6 , 2004 , we published an interim final rule in the Federal Register implementing the provisions of the Medicare Prescription Drug , Improvement , and Modernization Act of 2003 ( MMA ) related to the calculation and submission of manufacturer 's average sales price ( ASP ) data on certain Medicare Part B drugs and biologicals by manufacturers .
	manualset3
121058	7	404068	13	NULL	NULL	0	NULL	calculation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On April 6 , 2004 , we published an interim final rule in the Federal Register implementing the provisions of the Medicare Prescription Drug , Improvement , and Modernization Act of 2003 ( MMA ) related to the calculation and submission of manufacturer 's average sales price ( ASP ) data on certain Medicare Part B drugs and biologicals by manufacturers .
	manualset3
121059	8	404068	13	NULL	NULL	0	NULL	submission 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On April 6 , 2004 , we published an interim final rule in the Federal Register implementing the provisions of the Medicare Prescription Drug , Improvement , and Modernization Act of 2003 ( MMA ) related to the calculation and submission of manufacturer 's average sales price ( ASP ) data on certain Medicare Part B drugs and biologicals by manufacturers .
	manualset3
121060	9	404068	13	NULL	NULL	0	NULL	manufacturer 's	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	On April 6 , 2004 , we published an interim final rule in the Federal Register implementing the provisions of the Medicare Prescription Drug , Improvement , and Modernization Act of 2003 ( MMA ) related to the calculation and submission of manufacturer 's average sales price ( ASP ) data on certain Medicare Part B drugs and biologicals by manufacturers .
	manualset3
121061	10	404068	13	NULL	NULL	0	NULL	average sales price ( ASP ) data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	On April 6 , 2004 , we published an interim final rule in the Federal Register implementing the provisions of the Medicare Prescription Drug , Improvement , and Modernization Act of 2003 ( MMA ) related to the calculation and submission of manufacturer 's average sales price ( ASP ) data on certain Medicare Part B drugs and biologicals by manufacturers .
	manualset3
121062	11	404068	13	NULL	NULL	0	NULL	Medicare Part B drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	On April 6 , 2004 , we published an interim final rule in the Federal Register implementing the provisions of the Medicare Prescription Drug , Improvement , and Modernization Act of 2003 ( MMA ) related to the calculation and submission of manufacturer 's average sales price ( ASP ) data on certain Medicare Part B drugs and biologicals by manufacturers .
	manualset3
121063	12	404068	13	NULL	NULL	0	NULL	biologicals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On April 6 , 2004 , we published an interim final rule in the Federal Register implementing the provisions of the Medicare Prescription Drug , Improvement , and Modernization Act of 2003 ( MMA ) related to the calculation and submission of manufacturer 's average sales price ( ASP ) data on certain Medicare Part B drugs and biologicals by manufacturers .
	manualset3
121064	13	404068	13	NULL	NULL	0	NULL	manufacturers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On April 6 , 2004 , we published an interim final rule in the Federal Register implementing the provisions of the Medicare Prescription Drug , Improvement , and Modernization Act of 2003 ( MMA ) related to the calculation and submission of manufacturer 's average sales price ( ASP ) data on certain Medicare Part B drugs and biologicals by manufacturers .
	manualset3
121065	1	404069	13	NULL	NULL	0	NULL	D56	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	On D56 , the PI was reduced in the miUH .
	manualset3
121066	2	404069	13	NULL	NULL	0	NULL	PI	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On D56 , the PI was reduced in the miUH .
	manualset3
121067	3	404069	13	NULL	NULL	0	NULL	miUH	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	On D56 , the PI was reduced in the miUH .
	manualset3
121068	1	404070	13	NULL	NULL	0	NULL	Day 14	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	On Day 14 , each intermediate region produced over 70 % as much estrogen as the disc region .
	manualset3
121069	2	404070	13	NULL	NULL	0	NULL	intermediate region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	On Day 14 , each intermediate region produced over 70 % as much estrogen as the disc region .
	manualset3
121070	3	404070	13	NULL	NULL	0	NULL	70 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On Day 14 , each intermediate region produced over 70 % as much estrogen as the disc region .
	manualset3
121071	4	404070	13	NULL	NULL	0	NULL	estrogen	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On Day 14 , each intermediate region produced over 70 % as much estrogen as the disc region .
	manualset3
121072	5	404070	13	NULL	NULL	0	NULL	disc region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	On Day 14 , each intermediate region produced over 70 % as much estrogen as the disc region .
	manualset3
121073	1	404071	13	NULL	NULL	0	NULL	Day 23 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	On Day 23 both prolactin and PG induced significant elevations in plasma progesterone , but luteolysis did not occur .
	manualset3
121074	2	404071	13	NULL	NULL	0	NULL	prolactin 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On Day 23 both prolactin and PG induced significant elevations in plasma progesterone , but luteolysis did not occur .
	manualset3
121075	3	404071	13	NULL	NULL	0	NULL	PG 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On Day 23 both prolactin and PG induced significant elevations in plasma progesterone , but luteolysis did not occur .
	manualset3
121076	4	404071	13	NULL	NULL	0	NULL	significant elevations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On Day 23 both prolactin and PG induced significant elevations in plasma progesterone , but luteolysis did not occur .
	manualset3
121077	5	404071	13	NULL	NULL	0	NULL	plasma progesterone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On Day 23 both prolactin and PG induced significant elevations in plasma progesterone , but luteolysis did not occur .
	manualset3
121078	6	404071	13	NULL	NULL	0	NULL	luteolysis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On Day 23 both prolactin and PG induced significant elevations in plasma progesterone , but luteolysis did not occur .
	manualset3
121079	1	404072	13	NULL	NULL	0	NULL	Hs578T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	On Hs578T cells , IGFBP-3 bound to caveolin-1 and beta1-integrins , enhancing their aggregation , the recruitment of focal adhesion kinase , and the activation of MAPK .
	manualset3
121080	2	404072	13	NULL	NULL	0	NULL	IGFBP-3 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	On Hs578T cells , IGFBP-3 bound to caveolin-1 and beta1-integrins , enhancing their aggregation , the recruitment of focal adhesion kinase , and the activation of MAPK .
	manualset3
121081	3	404072	13	NULL	NULL	0	NULL	caveolin-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	On Hs578T cells , IGFBP-3 bound to caveolin-1 and beta1-integrins , enhancing their aggregation , the recruitment of focal adhesion kinase , and the activation of MAPK .
	manualset3
121082	4	404072	13	NULL	NULL	0	NULL	beta1-integrins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On Hs578T cells , IGFBP-3 bound to caveolin-1 and beta1-integrins , enhancing their aggregation , the recruitment of focal adhesion kinase , and the activation of MAPK .
	manualset3
121083	5	404072	13	NULL	NULL	0	NULL	aggregation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On Hs578T cells , IGFBP-3 bound to caveolin-1 and beta1-integrins , enhancing their aggregation , the recruitment of focal adhesion kinase , and the activation of MAPK .
	manualset3
121084	6	404072	13	NULL	NULL	0	NULL	recruitment 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On Hs578T cells , IGFBP-3 bound to caveolin-1 and beta1-integrins , enhancing their aggregation , the recruitment of focal adhesion kinase , and the activation of MAPK .
	manualset3
121085	7	404072	13	NULL	NULL	0	NULL	focal adhesion kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	On Hs578T cells , IGFBP-3 bound to caveolin-1 and beta1-integrins , enhancing their aggregation , the recruitment of focal adhesion kinase , and the activation of MAPK .
	manualset3
121086	8	404072	13	NULL	NULL	0	NULL	activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On Hs578T cells , IGFBP-3 bound to caveolin-1 and beta1-integrins , enhancing their aggregation , the recruitment of focal adhesion kinase , and the activation of MAPK .
	manualset3
121087	9	404072	13	NULL	NULL	0	NULL	MAPK 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	On Hs578T cells , IGFBP-3 bound to caveolin-1 and beta1-integrins , enhancing their aggregation , the recruitment of focal adhesion kinase , and the activation of MAPK .
	manualset3
121088	1	404073	13	NULL	NULL	0	NULL	phase II study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	On a phase II study , 80 patients with low-grade , transformed , or mantle cell lymphoma received ABMT with 4-hydroperoxycyclophosphamide ( 4-HC ) purging as part of initial or salvage therapy .
	manualset3
121089	2	404073	13	NULL	NULL	0	NULL	80	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On a phase II study , 80 patients with low-grade , transformed , or mantle cell lymphoma received ABMT with 4-hydroperoxycyclophosphamide ( 4-HC ) purging as part of initial or salvage therapy .
	manualset3
121090	3	404073	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On a phase II study , 80 patients with low-grade , transformed , or mantle cell lymphoma received ABMT with 4-hydroperoxycyclophosphamide ( 4-HC ) purging as part of initial or salvage therapy .
	manualset3
121091	4	404073	13	NULL	NULL	0	NULL	low-grade , transformed , or mantle cell lymphoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On a phase II study , 80 patients with low-grade , transformed , or mantle cell lymphoma received ABMT with 4-hydroperoxycyclophosphamide ( 4-HC ) purging as part of initial or salvage therapy .
	manualset3
121092	5	404073	13	NULL	NULL	0	NULL	ABMT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	On a phase II study , 80 patients with low-grade , transformed , or mantle cell lymphoma received ABMT with 4-hydroperoxycyclophosphamide ( 4-HC ) purging as part of initial or salvage therapy .
	manualset3
121093	6	404073	13	NULL	NULL	0	NULL	4-hydroperoxycyclophosphamide ( 4-HC ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On a phase II study , 80 patients with low-grade , transformed , or mantle cell lymphoma received ABMT with 4-hydroperoxycyclophosphamide ( 4-HC ) purging as part of initial or salvage therapy .
	manualset3
121094	7	404073	13	NULL	NULL	0	NULL	part of initial therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	On a phase II study , 80 patients with low-grade , transformed , or mantle cell lymphoma received ABMT with 4-hydroperoxycyclophosphamide ( 4-HC ) purging as part of initial or salvage therapy .
	manualset3
121095	8	404073	13	NULL	NULL	0	NULL	salvage therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	On a phase II study , 80 patients with low-grade , transformed , or mantle cell lymphoma received ABMT with 4-hydroperoxycyclophosphamide ( 4-HC ) purging as part of initial or salvage therapy .
	manualset3
121096	1	404074	13	NULL	NULL	0	NULL	Bw35 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A decrease of Bw35 in the whole sample , more prominent in those without brain atrophy , again failed to be significant after multiplying the probability by the number of antigens studied .
	manualset3
121097	2	404074	13	NULL	NULL	0	NULL	decrease 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A decrease of Bw35 in the whole sample , more prominent in those without brain atrophy , again failed to be significant after multiplying the probability by the number of antigens studied .
	manualset3
121098	3	404074	13	NULL	NULL	0	NULL	whole sample	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A decrease of Bw35 in the whole sample , more prominent in those without brain atrophy , again failed to be significant after multiplying the probability by the number of antigens studied .
	manualset3
121099	4	404074	13	NULL	NULL	0	NULL	brain atrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A decrease of Bw35 in the whole sample , more prominent in those without brain atrophy , again failed to be significant after multiplying the probability by the number of antigens studied .
	manualset3
121100	5	404074	13	NULL	NULL	0	NULL	probability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A decrease of Bw35 in the whole sample , more prominent in those without brain atrophy , again failed to be significant after multiplying the probability by the number of antigens studied .
	manualset3
121101	6	404074	13	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A decrease of Bw35 in the whole sample , more prominent in those without brain atrophy , again failed to be significant after multiplying the probability by the number of antigens studied .
	manualset3
121102	7	404074	13	NULL	NULL	0	NULL	antigens	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A decrease of Bw35 in the whole sample , more prominent in those without brain atrophy , again failed to be significant after multiplying the probability by the number of antigens studied .
	manualset3
121103	1	404075	13	NULL	NULL	0	NULL	admission	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On admission , he had a severe normocytic normochromic anemia ( hemoglobin 7.5 g/dl ) requiring a blood transfusion .
	manualset3
121104	2	404075	13	NULL	NULL	0	NULL	severe normocytic normochromic anemia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On admission , he had a severe normocytic normochromic anemia ( hemoglobin 7.5 g/dl ) requiring a blood transfusion .
	manualset3
121105	3	404075	13	NULL	NULL	0	NULL	hemoglobin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	On admission , he had a severe normocytic normochromic anemia ( hemoglobin 7.5 g/dl ) requiring a blood transfusion .
	manualset3
121106	4	404075	13	NULL	NULL	0	NULL	7.5 g/dl 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On admission , he had a severe normocytic normochromic anemia ( hemoglobin 7.5 g/dl ) requiring a blood transfusion .
	manualset3
121107	5	404075	13	NULL	NULL	0	NULL	blood transfusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	On admission , he had a severe normocytic normochromic anemia ( hemoglobin 7.5 g/dl ) requiring a blood transfusion .
	manualset3
121108	1	404076	13	NULL	NULL	0	NULL	30 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On average , at least 30 % of the herd had to be seropositive before the BTM ELISA was found positive for lungworm antibodies .
	manualset3
121109	2	404076	13	NULL	NULL	0	NULL	herd	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On average , at least 30 % of the herd had to be seropositive before the BTM ELISA was found positive for lungworm antibodies .
	manualset3
121110	3	404076	13	NULL	NULL	0	NULL	BTM ELISA 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	On average , at least 30 % of the herd had to be seropositive before the BTM ELISA was found positive for lungworm antibodies .
	manualset3
121111	4	404076	13	NULL	NULL	0	NULL	lungworm antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On average , at least 30 % of the herd had to be seropositive before the BTM ELISA was found positive for lungworm antibodies .
	manualset3
121112	1	404077	13	NULL	NULL	0	NULL	CVM samples 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On average , more CVM samples were positive for T. fetus for a longer period of time in the control than in the vaccinated heifers ( 3.9 vs 1.85 sampling periods , respectively ; P & lt ; 0.08 ) .
	manualset3
121113	2	404077	13	NULL	NULL	0	NULL	T. fetus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On average , more CVM samples were positive for T. fetus for a longer period of time in the control than in the vaccinated heifers ( 3.9 vs 1.85 sampling periods , respectively ; P & lt ; 0.08 ) .
	manualset3
121114	3	404077	13	NULL	NULL	0	NULL	longer period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	On average , more CVM samples were positive for T. fetus for a longer period of time in the control than in the vaccinated heifers ( 3.9 vs 1.85 sampling periods , respectively ; P & lt ; 0.08 ) .
	manualset3
121115	4	404077	13	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	On average , more CVM samples were positive for T. fetus for a longer period of time in the control than in the vaccinated heifers ( 3.9 vs 1.85 sampling periods , respectively ; P & lt ; 0.08 ) .
	manualset3
121116	5	404077	13	NULL	NULL	0	NULL	control	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On average , more CVM samples were positive for T. fetus for a longer period of time in the control than in the vaccinated heifers ( 3.9 vs 1.85 sampling periods , respectively ; P & lt ; 0.08 ) .
	manualset3
121117	6	404077	13	NULL	NULL	0	NULL	vaccinated heifers 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On average , more CVM samples were positive for T. fetus for a longer period of time in the control than in the vaccinated heifers ( 3.9 vs 1.85 sampling periods , respectively ; P & lt ; 0.08 ) .
	manualset3
121118	7	404077	13	NULL	NULL	0	NULL	3.9 sampling periods	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	On average , more CVM samples were positive for T. fetus for a longer period of time in the control than in the vaccinated heifers ( 3.9 vs 1.85 sampling periods , respectively ; P & lt ; 0.08 ) .
	manualset3
121119	8	404077	13	NULL	NULL	0	NULL	1.85 sampling periods	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	On average , more CVM samples were positive for T. fetus for a longer period of time in the control than in the vaccinated heifers ( 3.9 vs 1.85 sampling periods , respectively ; P & lt ; 0.08 ) .
	manualset3
121120	9	404077	13	NULL	NULL	0	NULL	P & lt ; 0.08	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On average , more CVM samples were positive for T. fetus for a longer period of time in the control than in the vaccinated heifers ( 3.9 vs 1.85 sampling periods , respectively ; P & lt ; 0.08 ) .
	manualset3
121121	1	404078	13	NULL	NULL	0	NULL	tissues 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	On both tissues , penetration by the pathogen occurred from appressoria and host colonization was first subcuticular and then intracellular .
	manualset3
121122	2	404078	13	NULL	NULL	0	NULL	penetration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On both tissues , penetration by the pathogen occurred from appressoria and host colonization was first subcuticular and then intracellular .
	manualset3
121123	3	404078	13	NULL	NULL	0	NULL	pathogen	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On both tissues , penetration by the pathogen occurred from appressoria and host colonization was first subcuticular and then intracellular .
	manualset3
121124	4	404078	13	NULL	NULL	0	NULL	appressoria	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	On both tissues , penetration by the pathogen occurred from appressoria and host colonization was first subcuticular and then intracellular .
	manualset3
121125	5	404078	13	NULL	NULL	0	NULL	host 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On both tissues , penetration by the pathogen occurred from appressoria and host colonization was first subcuticular and then intracellular .
	manualset3
121126	6	404078	13	NULL	NULL	0	NULL	colonization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On both tissues , penetration by the pathogen occurred from appressoria and host colonization was first subcuticular and then intracellular .
	manualset3
121127	1	404079	13	NULL	NULL	0	NULL	completion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On completion , three patients began treatment with Naltrexone and another was abstinent at a follow-up appointment , 1 week later .
	manualset3
121128	2	404079	13	NULL	NULL	0	NULL	three patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On completion , three patients began treatment with Naltrexone and another was abstinent at a follow-up appointment , 1 week later .
	manualset3
121129	3	404079	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	On completion , three patients began treatment with Naltrexone and another was abstinent at a follow-up appointment , 1 week later .
	manualset3
121130	4	404079	13	NULL	NULL	0	NULL	Naltrexone 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	On completion , three patients began treatment with Naltrexone and another was abstinent at a follow-up appointment , 1 week later .
	manualset3
121131	5	404079	13	NULL	NULL	0	NULL	follow-up appointment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	On completion , three patients began treatment with Naltrexone and another was abstinent at a follow-up appointment , 1 week later .
	manualset3
121132	6	404079	13	NULL	NULL	NULL	NULL	1 week	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On completion , three patients began treatment with Naltrexone and another was abstinent at a follow-up appointment , 1 week later .
	manualset3
121133	1	404080	13	NULL	NULL	0	NULL	constitutive relations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On constitutive relations and finite deformations of passive cardiac tissue : I. A pseudostrain-energy function .
	manualset3
121134	2	404080	13	NULL	NULL	0	NULL	finite deformations 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On constitutive relations and finite deformations of passive cardiac tissue : I. A pseudostrain-energy function .
	manualset3
121135	3	404080	13	NULL	NULL	0	NULL	passive cardiac tissue 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	On constitutive relations and finite deformations of passive cardiac tissue : I. A pseudostrain-energy function .
	manualset3
121136	4	404080	13	NULL	NULL	0	NULL	 pseudostrain-energy function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On constitutive relations and finite deformations of passive cardiac tissue : I. A pseudostrain-energy function .
	manualset3
121137	1	404081	13	NULL	NULL	0	NULL	day 17 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 17 , heifers and cows received additional PGF2alpha and follicular fluids from preovulatory follicles were collected on day 19 perior to the expected estrus .
	manualset3
121138	2	404081	13	NULL	NULL	0	NULL	heifers	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 17 , heifers and cows received additional PGF2alpha and follicular fluids from preovulatory follicles were collected on day 19 perior to the expected estrus .
	manualset3
121139	3	404081	13	NULL	NULL	0	NULL	cows	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 17 , heifers and cows received additional PGF2alpha and follicular fluids from preovulatory follicles were collected on day 19 perior to the expected estrus .
	manualset3
121140	4	404081	13	NULL	NULL	0	NULL	PGF2alpha	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 17 , heifers and cows received additional PGF2alpha and follicular fluids from preovulatory follicles were collected on day 19 perior to the expected estrus .
	manualset3
121141	5	404081	13	NULL	NULL	0	NULL	follicular fluids 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 17 , heifers and cows received additional PGF2alpha and follicular fluids from preovulatory follicles were collected on day 19 perior to the expected estrus .
	manualset3
121142	6	404081	13	NULL	NULL	0	NULL	preovulatory follicles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 17 , heifers and cows received additional PGF2alpha and follicular fluids from preovulatory follicles were collected on day 19 perior to the expected estrus .
	manualset3
121143	7	404081	13	NULL	NULL	0	NULL	day 19	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 17 , heifers and cows received additional PGF2alpha and follicular fluids from preovulatory follicles were collected on day 19 perior to the expected estrus .
	manualset3
125241	8	404081	13	NULL	NULL	0	NULL	estrus	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 17 , heifers and cows received additional PGF2alpha and follicular fluids from preovulatory follicles were collected on day 19 perior to the expected estrus .
	manualset3
121144	1	404082	13	NULL	NULL	0	NULL	day 3	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 3 , a reduction of viral clearance was shown by the presence of elevated viral titers and viral replication in the heart of IL-6TG .
	manualset3
121145	2	404082	13	NULL	NULL	0	NULL	reduction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 3 , a reduction of viral clearance was shown by the presence of elevated viral titers and viral replication in the heart of IL-6TG .
	manualset3
121146	3	404082	13	NULL	NULL	0	NULL	viral clearance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 3 , a reduction of viral clearance was shown by the presence of elevated viral titers and viral replication in the heart of IL-6TG .
	manualset3
121147	4	404082	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 3 , a reduction of viral clearance was shown by the presence of elevated viral titers and viral replication in the heart of IL-6TG .
	manualset3
121148	5	404082	13	NULL	NULL	0	NULL	viral titers 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 3 , a reduction of viral clearance was shown by the presence of elevated viral titers and viral replication in the heart of IL-6TG .
	manualset3
121149	6	404082	13	NULL	NULL	0	NULL	viral replication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 3 , a reduction of viral clearance was shown by the presence of elevated viral titers and viral replication in the heart of IL-6TG .
	manualset3
121150	7	404082	13	NULL	NULL	0	NULL	heart	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 3 , a reduction of viral clearance was shown by the presence of elevated viral titers and viral replication in the heart of IL-6TG .
	manualset3
121151	8	404082	13	NULL	NULL	0	NULL	IL-6TG	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 3 , a reduction of viral clearance was shown by the presence of elevated viral titers and viral replication in the heart of IL-6TG .
	manualset3
121152	1	404083	13	NULL	NULL	0	NULL	day 30	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 30 , mast cells could not be distinguished from those in adult rats .
	manualset3
121153	2	404083	13	NULL	NULL	0	NULL	mast cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 30 , mast cells could not be distinguished from those in adult rats .
	manualset3
121154	3	404083	13	NULL	NULL	0	NULL	adult rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 30 , mast cells could not be distinguished from those in adult rats .
	manualset3
121155	1	404084	13	NULL	NULL	0	NULL	day 30 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 30 after germination , Na-deficient A. tricolor plants received either 0.5 millimolar NaCl or KCl .
	manualset3
121156	2	404084	13	NULL	NULL	0	NULL	germination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 30 after germination , Na-deficient A. tricolor plants received either 0.5 millimolar NaCl or KCl .
	manualset3
121157	3	404084	13	NULL	NULL	0	NULL	Na-deficient A. tricolor plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 30 after germination , Na-deficient A. tricolor plants received either 0.5 millimolar NaCl or KCl .
	manualset3
121158	4	404084	13	NULL	NULL	0	NULL	0.5 millimolar 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 30 after germination , Na-deficient A. tricolor plants received either 0.5 millimolar NaCl or KCl .
	manualset3
121159	5	404084	13	NULL	NULL	0	NULL	NaCl 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 30 after germination , Na-deficient A. tricolor plants received either 0.5 millimolar NaCl or KCl .
	manualset3
121160	6	404084	13	NULL	NULL	0	NULL	KCl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 30 after germination , Na-deficient A. tricolor plants received either 0.5 millimolar NaCl or KCl .
	manualset3
121161	1	404085	13	NULL	NULL	0	NULL	day 7	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 7 , 14 and 21 after BMT , the expressions of bFGF mRNA and protein in bone marrow stromal cells of ligustrazine group and saline group were lower than that in bone marrow stromal cells of normal group , but the expressions of bFGF mRNA and protein in ligustrazine group were obviously higher than that in saline group ( P & lt ; 0.01 or P & lt ; 0.05 ) .
	manualset3
121162	2	404085	13	NULL	NULL	0	NULL	day 14	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 7 , 14 and 21 after BMT , the expressions of bFGF mRNA and protein in bone marrow stromal cells of ligustrazine group and saline group were lower than that in bone marrow stromal cells of normal group , but the expressions of bFGF mRNA and protein in ligustrazine group were obviously higher than that in saline group ( P & lt ; 0.01 or P & lt ; 0.05 ) .
	manualset3
121163	3	404085	13	NULL	NULL	0	NULL	day 21	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 7 , 14 and 21 after BMT , the expressions of bFGF mRNA and protein in bone marrow stromal cells of ligustrazine group and saline group were lower than that in bone marrow stromal cells of normal group , but the expressions of bFGF mRNA and protein in ligustrazine group were obviously higher than that in saline group ( P & lt ; 0.01 or P & lt ; 0.05 ) .
	manualset3
121164	4	404085	13	NULL	NULL	0	NULL	BMT 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 7 , 14 and 21 after BMT , the expressions of bFGF mRNA and protein in bone marrow stromal cells of ligustrazine group and saline group were lower than that in bone marrow stromal cells of normal group , but the expressions of bFGF mRNA and protein in ligustrazine group were obviously higher than that in saline group ( P & lt ; 0.01 or P & lt ; 0.05 ) .
	manualset3
121165	5	404085	13	NULL	NULL	0	NULL	expressions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 7 , 14 and 21 after BMT , the expressions of bFGF mRNA and protein in bone marrow stromal cells of ligustrazine group and saline group were lower than that in bone marrow stromal cells of normal group , but the expressions of bFGF mRNA and protein in ligustrazine group were obviously higher than that in saline group ( P & lt ; 0.01 or P & lt ; 0.05 ) .
	manualset3
121166	6	404085	13	NULL	NULL	0	NULL	bFGF mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 7 , 14 and 21 after BMT , the expressions of bFGF mRNA and protein in bone marrow stromal cells of ligustrazine group and saline group were lower than that in bone marrow stromal cells of normal group , but the expressions of bFGF mRNA and protein in ligustrazine group were obviously higher than that in saline group ( P & lt ; 0.01 or P & lt ; 0.05 ) .
	manualset3
121167	7	404085	13	NULL	NULL	0	NULL	bFGF protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 7 , 14 and 21 after BMT , the expressions of bFGF mRNA and protein in bone marrow stromal cells of ligustrazine group and saline group were lower than that in bone marrow stromal cells of normal group , but the expressions of bFGF mRNA and protein in ligustrazine group were obviously higher than that in saline group ( P & lt ; 0.01 or P & lt ; 0.05 ) .
	manualset3
121168	8	404085	13	NULL	NULL	0	NULL	bone marrow stromal cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 7 , 14 and 21 after BMT , the expressions of bFGF mRNA and protein in bone marrow stromal cells of ligustrazine group and saline group were lower than that in bone marrow stromal cells of normal group , but the expressions of bFGF mRNA and protein in ligustrazine group were obviously higher than that in saline group ( P & lt ; 0.01 or P & lt ; 0.05 ) .
	manualset3
121169	9	404085	13	NULL	NULL	NULL	NULL	ligustrazine group	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On day 7 , 14 and 21 after BMT , the expressions of bFGF mRNA and protein in bone marrow stromal cells of ligustrazine group and saline group were lower than that in bone marrow stromal cells of normal group , but the expressions of bFGF mRNA and protein in ligustrazine group were obviously higher than that in saline group ( P & lt ; 0.01 or P & lt ; 0.05 ) .
	manualset3
121170	10	404085	13	NULL	NULL	NULL	NULL	saline group	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On day 7 , 14 and 21 after BMT , the expressions of bFGF mRNA and protein in bone marrow stromal cells of ligustrazine group and saline group were lower than that in bone marrow stromal cells of normal group , but the expressions of bFGF mRNA and protein in ligustrazine group were obviously higher than that in saline group ( P & lt ; 0.01 or P & lt ; 0.05 ) .
	manualset3
121171	11	404085	13	NULL	NULL	0	NULL	bone marrow stromal cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 7 , 14 and 21 after BMT , the expressions of bFGF mRNA and protein in bone marrow stromal cells of ligustrazine group and saline group were lower than that in bone marrow stromal cells of normal group , but the expressions of bFGF mRNA and protein in ligustrazine group were obviously higher than that in saline group ( P & lt ; 0.01 or P & lt ; 0.05 ) .
	manualset3
121172	12	404085	13	NULL	NULL	0	NULL	expressions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 7 , 14 and 21 after BMT , the expressions of bFGF mRNA and protein in bone marrow stromal cells of ligustrazine group and saline group were lower than that in bone marrow stromal cells of normal group , but the expressions of bFGF mRNA and protein in ligustrazine group were obviously higher than that in saline group ( P & lt ; 0.01 or P & lt ; 0.05 ) .
	manualset3
121173	13	404085	13	NULL	NULL	0	NULL	bFGF mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 7 , 14 and 21 after BMT , the expressions of bFGF mRNA and protein in bone marrow stromal cells of ligustrazine group and saline group were lower than that in bone marrow stromal cells of normal group , but the expressions of bFGF mRNA and protein in ligustrazine group were obviously higher than that in saline group ( P & lt ; 0.01 or P & lt ; 0.05 ) .
	manualset3
121174	14	404085	13	NULL	NULL	0	NULL	bFGF protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 7 , 14 and 21 after BMT , the expressions of bFGF mRNA and protein in bone marrow stromal cells of ligustrazine group and saline group were lower than that in bone marrow stromal cells of normal group , but the expressions of bFGF mRNA and protein in ligustrazine group were obviously higher than that in saline group ( P & lt ; 0.01 or P & lt ; 0.05 ) .
	manualset3
121175	15	404085	13	NULL	NULL	0	NULL	ligustrazine group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 7 , 14 and 21 after BMT , the expressions of bFGF mRNA and protein in bone marrow stromal cells of ligustrazine group and saline group were lower than that in bone marrow stromal cells of normal group , but the expressions of bFGF mRNA and protein in ligustrazine group were obviously higher than that in saline group ( P & lt ; 0.01 or P & lt ; 0.05 ) .
	manualset3
121176	16	404085	13	NULL	NULL	0	NULL	saline group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 7 , 14 and 21 after BMT , the expressions of bFGF mRNA and protein in bone marrow stromal cells of ligustrazine group and saline group were lower than that in bone marrow stromal cells of normal group , but the expressions of bFGF mRNA and protein in ligustrazine group were obviously higher than that in saline group ( P & lt ; 0.01 or P & lt ; 0.05 ) .
	manualset3
121177	17	404085	13	NULL	NULL	0	NULL	P & lt ; 0.01 or P & lt ; 0.05 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 7 , 14 and 21 after BMT , the expressions of bFGF mRNA and protein in bone marrow stromal cells of ligustrazine group and saline group were lower than that in bone marrow stromal cells of normal group , but the expressions of bFGF mRNA and protein in ligustrazine group were obviously higher than that in saline group ( P & lt ; 0.01 or P & lt ; 0.05 ) .
	manualset3
121178	1	404086	13	NULL	NULL	0	NULL	day seven	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	On day seven after institution of the 'EM A ' regimen ( etoposide , medium dose methotrexate with folinic acid rescue and actinomycin-D ) , complete pneumothorax occurred .
	manualset3
121179	2	404086	13	NULL	NULL	0	NULL	institution	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	On day seven after institution of the 'EM A ' regimen ( etoposide , medium dose methotrexate with folinic acid rescue and actinomycin-D ) , complete pneumothorax occurred .
	manualset3
121180	3	404086	13	NULL	NULL	0	NULL	'EM A ' regimen 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	On day seven after institution of the 'EM A ' regimen ( etoposide , medium dose methotrexate with folinic acid rescue and actinomycin-D ) , complete pneumothorax occurred .
	manualset3
121181	4	404086	13	NULL	NULL	0	NULL	etoposide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	On day seven after institution of the 'EM A ' regimen ( etoposide , medium dose methotrexate with folinic acid rescue and actinomycin-D ) , complete pneumothorax occurred .
	manualset3
121182	5	404086	13	NULL	NULL	NULL	NULL	medium dose 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On day seven after institution of the 'EM A ' regimen ( etoposide , medium dose methotrexate with folinic acid rescue and actinomycin-D ) , complete pneumothorax occurred .
	manualset3
121183	6	404086	13	NULL	NULL	0	NULL	methotrexate	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	On day seven after institution of the 'EM A ' regimen ( etoposide , medium dose methotrexate with folinic acid rescue and actinomycin-D ) , complete pneumothorax occurred .
	manualset3
121184	7	404086	13	NULL	NULL	0	NULL	folinic acid rescue 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	On day seven after institution of the 'EM A ' regimen ( etoposide , medium dose methotrexate with folinic acid rescue and actinomycin-D ) , complete pneumothorax occurred .
	manualset3
121185	8	404086	13	NULL	NULL	0	NULL	actinomycin-D	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	On day seven after institution of the 'EM A ' regimen ( etoposide , medium dose methotrexate with folinic acid rescue and actinomycin-D ) , complete pneumothorax occurred .
	manualset3
121186	9	404086	13	NULL	NULL	0	NULL	pneumothorax 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	On day seven after institution of the 'EM A ' regimen ( etoposide , medium dose methotrexate with folinic acid rescue and actinomycin-D ) , complete pneumothorax occurred .
	manualset3
121187	1	404087	13	NULL	NULL	NULL	NULL	examination	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On examination , he had decreased corneal diameter and corectopia of the right eye ( OD ) , without any noteworthy findings on the biomicroscopy of the left eye ( OS ) .
	manualset3
121188	2	404087	13	NULL	NULL	0	NULL	corneal diameter	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On examination , he had decreased corneal diameter and corectopia of the right eye ( OD ) , without any noteworthy findings on the biomicroscopy of the left eye ( OS ) .
	manualset3
121189	3	404087	13	NULL	NULL	0	NULL	corectopia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On examination , he had decreased corneal diameter and corectopia of the right eye ( OD ) , without any noteworthy findings on the biomicroscopy of the left eye ( OS ) .
	manualset3
121190	4	404087	13	NULL	NULL	NULL	NULL	right eye ( OD ) 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On examination , he had decreased corneal diameter and corectopia of the right eye ( OD ) , without any noteworthy findings on the biomicroscopy of the left eye ( OS ) .
	manualset3
121191	5	404087	13	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On examination , he had decreased corneal diameter and corectopia of the right eye ( OD ) , without any noteworthy findings on the biomicroscopy of the left eye ( OS ) .
	manualset3
121192	6	404087	13	NULL	NULL	0	NULL	biomicroscopy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	On examination , he had decreased corneal diameter and corectopia of the right eye ( OD ) , without any noteworthy findings on the biomicroscopy of the left eye ( OS ) .
	manualset3
121193	7	404087	13	NULL	NULL	0	NULL	left eye ( OS )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	On examination , he had decreased corneal diameter and corectopia of the right eye ( OD ) , without any noteworthy findings on the biomicroscopy of the left eye ( OS ) .
	manualset3
121194	1	404088	13	NULL	NULL	0	NULL	examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	On examination , she had moderately severe fatigable proximal muscle weakness and ptosis .
	manualset3
121195	2	404088	13	NULL	NULL	0	NULL	proximal muscle weakness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On examination , she had moderately severe fatigable proximal muscle weakness and ptosis .
	manualset3
121196	3	404088	13	NULL	NULL	0	NULL	ptosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On examination , she had moderately severe fatigable proximal muscle weakness and ptosis .
	manualset3
121197	1	404089	13	NULL	NULL	0	NULL	fishing expeditions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On fishing expeditions , laws of fishing , and good fishermen .
	manualset3
121198	2	404089	13	NULL	NULL	0	NULL	laws of fishing	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	On fishing expeditions , laws of fishing , and good fishermen .
	manualset3
121199	3	404089	13	NULL	NULL	0	NULL	good fishermen	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On fishing expeditions , laws of fishing , and good fishermen .
	manualset3
121200	1	404090	13	NULL	NULL	0	NULL	histological examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	On histological examination , epithelial damage in the trachea and peripheral airways was recognized after ozone exposure .
	manualset3
121201	2	404090	13	NULL	NULL	0	NULL	epithelial damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On histological examination , epithelial damage in the trachea and peripheral airways was recognized after ozone exposure .
	manualset3
121202	3	404090	13	NULL	NULL	0	NULL	trachea	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	On histological examination , epithelial damage in the trachea and peripheral airways was recognized after ozone exposure .
	manualset3
121203	4	404090	13	NULL	NULL	0	NULL	peripheral airways	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	On histological examination , epithelial damage in the trachea and peripheral airways was recognized after ozone exposure .
	manualset3
121204	5	404090	13	NULL	NULL	0	NULL	ozone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On histological examination , epithelial damage in the trachea and peripheral airways was recognized after ozone exposure .
	manualset3
121205	6	404090	13	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On histological examination , epithelial damage in the trachea and peripheral airways was recognized after ozone exposure .
	manualset3
121206	1	404091	13	NULL	NULL	0	NULL	incubation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On incubation with ( 32P ) NAD or ( 14C ) NAD , modification of the adenovirus T antigen could be demonstrated in one of these systems .
	manualset3
121207	2	404091	13	NULL	NULL	0	NULL	( 32P ) NAD	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On incubation with ( 32P ) NAD or ( 14C ) NAD , modification of the adenovirus T antigen could be demonstrated in one of these systems .
	manualset3
121208	3	404091	13	NULL	NULL	0	NULL	( 14C ) NAD	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On incubation with ( 32P ) NAD or ( 14C ) NAD , modification of the adenovirus T antigen could be demonstrated in one of these systems .
	manualset3
121209	4	404091	13	NULL	NULL	0	NULL	modification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On incubation with ( 32P ) NAD or ( 14C ) NAD , modification of the adenovirus T antigen could be demonstrated in one of these systems .
	manualset3
121210	5	404091	13	NULL	NULL	0	NULL	adenovirus T antigen	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On incubation with ( 32P ) NAD or ( 14C ) NAD , modification of the adenovirus T antigen could be demonstrated in one of these systems .
	manualset3
121211	6	404091	13	NULL	NULL	0	NULL	systems	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	On incubation with ( 32P ) NAD or ( 14C ) NAD , modification of the adenovirus T antigen could be demonstrated in one of these systems .
	manualset3
121212	1	404092	13	NULL	NULL	0	NULL	defect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A defect of kl gene expression in the mouse results in a syndrome resembling human aging , such as arteriosclerosis , skin atrophy , osteoporosis , and pulmonary emphysema .
	manualset3
121213	2	404092	13	NULL	NULL	0	NULL	kl gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A defect of kl gene expression in the mouse results in a syndrome resembling human aging , such as arteriosclerosis , skin atrophy , osteoporosis , and pulmonary emphysema .
	manualset3
121214	3	404092	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A defect of kl gene expression in the mouse results in a syndrome resembling human aging , such as arteriosclerosis , skin atrophy , osteoporosis , and pulmonary emphysema .
	manualset3
121215	4	404092	13	NULL	NULL	0	NULL	mouse	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A defect of kl gene expression in the mouse results in a syndrome resembling human aging , such as arteriosclerosis , skin atrophy , osteoporosis , and pulmonary emphysema .
	manualset3
121216	5	404092	13	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A defect of kl gene expression in the mouse results in a syndrome resembling human aging , such as arteriosclerosis , skin atrophy , osteoporosis , and pulmonary emphysema .
	manualset3
121217	6	404092	13	NULL	NULL	0	NULL	syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A defect of kl gene expression in the mouse results in a syndrome resembling human aging , such as arteriosclerosis , skin atrophy , osteoporosis , and pulmonary emphysema .
	manualset3
121218	7	404092	13	NULL	NULL	0	NULL	human aging	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A defect of kl gene expression in the mouse results in a syndrome resembling human aging , such as arteriosclerosis , skin atrophy , osteoporosis , and pulmonary emphysema .
	manualset3
121219	8	404092	13	NULL	NULL	0	NULL	arteriosclerosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A defect of kl gene expression in the mouse results in a syndrome resembling human aging , such as arteriosclerosis , skin atrophy , osteoporosis , and pulmonary emphysema .
	manualset3
121220	9	404092	13	NULL	NULL	0	NULL	skin atrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A defect of kl gene expression in the mouse results in a syndrome resembling human aging , such as arteriosclerosis , skin atrophy , osteoporosis , and pulmonary emphysema .
	manualset3
121221	10	404092	13	NULL	NULL	0	NULL	osteoporosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A defect of kl gene expression in the mouse results in a syndrome resembling human aging , such as arteriosclerosis , skin atrophy , osteoporosis , and pulmonary emphysema .
	manualset3
121222	11	404092	13	NULL	NULL	0	NULL	pulmonary emphysema	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A defect of kl gene expression in the mouse results in a syndrome resembling human aging , such as arteriosclerosis , skin atrophy , osteoporosis , and pulmonary emphysema .
	manualset3
121223	1	404093	13	NULL	NULL	0	NULL	knowledge	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On knowledge , policy , practice , and fate .
	manualset3
121224	2	404093	13	NULL	NULL	0	NULL	policy	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	On knowledge , policy , practice , and fate .
	manualset3
121225	3	404093	13	NULL	NULL	0	NULL	practice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On knowledge , policy , practice , and fate .
	manualset3
121226	4	404093	13	NULL	NULL	0	NULL	fate	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On knowledge , policy , practice , and fate .
	manualset3
121238	1	404094	13	NULL	NULL	0	NULL	multivariate analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	On multivariate analysis , only tumor size ( P & lt ; 0.05 ) , albumin ( P & lt ; 0.01 ) and systemic treatment ( P & lt ; 0.0001 ) were significant independent predictors of relapse-free , cancer-specific and overall survival .
	manualset3
121239	2	404094	13	NULL	NULL	0	NULL	tumor size 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On multivariate analysis , only tumor size ( P & lt ; 0.05 ) , albumin ( P & lt ; 0.01 ) and systemic treatment ( P & lt ; 0.0001 ) were significant independent predictors of relapse-free , cancer-specific and overall survival .
	manualset3
121240	3	404094	13	NULL	NULL	0	NULL	P & lt ; 0.05 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On multivariate analysis , only tumor size ( P & lt ; 0.05 ) , albumin ( P & lt ; 0.01 ) and systemic treatment ( P & lt ; 0.0001 ) were significant independent predictors of relapse-free , cancer-specific and overall survival .
	manualset3
121241	4	404094	13	NULL	NULL	0	NULL	albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	On multivariate analysis , only tumor size ( P & lt ; 0.05 ) , albumin ( P & lt ; 0.01 ) and systemic treatment ( P & lt ; 0.0001 ) were significant independent predictors of relapse-free , cancer-specific and overall survival .
	manualset3
121242	5	404094	13	NULL	NULL	0	NULL	P & lt ; 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On multivariate analysis , only tumor size ( P & lt ; 0.05 ) , albumin ( P & lt ; 0.01 ) and systemic treatment ( P & lt ; 0.0001 ) were significant independent predictors of relapse-free , cancer-specific and overall survival .
	manualset3
121243	6	404094	13	NULL	NULL	0	NULL	systemic treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	On multivariate analysis , only tumor size ( P & lt ; 0.05 ) , albumin ( P & lt ; 0.01 ) and systemic treatment ( P & lt ; 0.0001 ) were significant independent predictors of relapse-free , cancer-specific and overall survival .
	manualset3
121244	7	404094	13	NULL	NULL	0	NULL	P & lt ; 0.0001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On multivariate analysis , only tumor size ( P & lt ; 0.05 ) , albumin ( P & lt ; 0.01 ) and systemic treatment ( P & lt ; 0.0001 ) were significant independent predictors of relapse-free , cancer-specific and overall survival .
	manualset3
121245	8	404094	13	NULL	NULL	0	NULL	predictors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On multivariate analysis , only tumor size ( P & lt ; 0.05 ) , albumin ( P & lt ; 0.01 ) and systemic treatment ( P & lt ; 0.0001 ) were significant independent predictors of relapse-free , cancer-specific and overall survival .
	manualset3
121246	9	404094	13	NULL	NULL	0	NULL	survival 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On multivariate analysis , only tumor size ( P & lt ; 0.05 ) , albumin ( P & lt ; 0.01 ) and systemic treatment ( P & lt ; 0.0001 ) were significant independent predictors of relapse-free , cancer-specific and overall survival .
	manualset3
121247	1	404095	13	NULL	NULL	0	NULL	neuropsychological testing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	On neuropsychological testing , subjects with AIDS-related complex performed at a significantly lower level than the HIV-1 seronegative group ( p = 0.001 ) .
	manualset3
121248	2	404095	13	NULL	NULL	0	NULL	subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On neuropsychological testing , subjects with AIDS-related complex performed at a significantly lower level than the HIV-1 seronegative group ( p = 0.001 ) .
	manualset3
121249	3	404095	13	NULL	NULL	0	NULL	AIDS-related complex 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On neuropsychological testing , subjects with AIDS-related complex performed at a significantly lower level than the HIV-1 seronegative group ( p = 0.001 ) .
	manualset3
121250	4	404095	13	NULL	NULL	0	NULL	level	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On neuropsychological testing , subjects with AIDS-related complex performed at a significantly lower level than the HIV-1 seronegative group ( p = 0.001 ) .
	manualset3
121251	5	404095	13	NULL	NULL	0	NULL	HIV-1 seronegative group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On neuropsychological testing , subjects with AIDS-related complex performed at a significantly lower level than the HIV-1 seronegative group ( p = 0.001 ) .
	manualset3
121252	6	404095	13	NULL	NULL	0	NULL	p = 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On neuropsychological testing , subjects with AIDS-related complex performed at a significantly lower level than the HIV-1 seronegative group ( p = 0.001 ) .
	manualset3
121253	1	404096	13	NULL	NULL	0	NULL	occasion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On one occasion , exercise was preceded by whole-body cooling achieved by immersion in water during a reduction in temperature from 29 to 24 degrees C , and , for the other trial , by immersion in water at a thermoneutral temperature ( control , 34.8 degrees C ) .
	manualset3
121254	2	404096	13	NULL	NULL	0	NULL	exercise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On one occasion , exercise was preceded by whole-body cooling achieved by immersion in water during a reduction in temperature from 29 to 24 degrees C , and , for the other trial , by immersion in water at a thermoneutral temperature ( control , 34.8 degrees C ) .
	manualset3
121255	3	404096	13	NULL	NULL	0	NULL	cooling 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On one occasion , exercise was preceded by whole-body cooling achieved by immersion in water during a reduction in temperature from 29 to 24 degrees C , and , for the other trial , by immersion in water at a thermoneutral temperature ( control , 34.8 degrees C ) .
	manualset3
121256	4	404096	13	NULL	NULL	0	NULL	immersion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On one occasion , exercise was preceded by whole-body cooling achieved by immersion in water during a reduction in temperature from 29 to 24 degrees C , and , for the other trial , by immersion in water at a thermoneutral temperature ( control , 34.8 degrees C ) .
	manualset3
121257	5	404096	13	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On one occasion , exercise was preceded by whole-body cooling achieved by immersion in water during a reduction in temperature from 29 to 24 degrees C , and , for the other trial , by immersion in water at a thermoneutral temperature ( control , 34.8 degrees C ) .
	manualset3
121258	6	404096	13	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On one occasion , exercise was preceded by whole-body cooling achieved by immersion in water during a reduction in temperature from 29 to 24 degrees C , and , for the other trial , by immersion in water at a thermoneutral temperature ( control , 34.8 degrees C ) .
	manualset3
121259	7	404096	13	NULL	NULL	0	NULL	temperature 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On one occasion , exercise was preceded by whole-body cooling achieved by immersion in water during a reduction in temperature from 29 to 24 degrees C , and , for the other trial , by immersion in water at a thermoneutral temperature ( control , 34.8 degrees C ) .
	manualset3
121260	8	404096	13	NULL	NULL	0	NULL	29 to 24 degrees C 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On one occasion , exercise was preceded by whole-body cooling achieved by immersion in water during a reduction in temperature from 29 to 24 degrees C , and , for the other trial , by immersion in water at a thermoneutral temperature ( control , 34.8 degrees C ) .
	manualset3
121261	9	404096	13	NULL	NULL	0	NULL	trial	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	On one occasion , exercise was preceded by whole-body cooling achieved by immersion in water during a reduction in temperature from 29 to 24 degrees C , and , for the other trial , by immersion in water at a thermoneutral temperature ( control , 34.8 degrees C ) .
	manualset3
121262	10	404096	13	NULL	NULL	0	NULL	immersion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On one occasion , exercise was preceded by whole-body cooling achieved by immersion in water during a reduction in temperature from 29 to 24 degrees C , and , for the other trial , by immersion in water at a thermoneutral temperature ( control , 34.8 degrees C ) .
	manualset3
121263	11	404096	13	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On one occasion , exercise was preceded by whole-body cooling achieved by immersion in water during a reduction in temperature from 29 to 24 degrees C , and , for the other trial , by immersion in water at a thermoneutral temperature ( control , 34.8 degrees C ) .
	manualset3
121264	12	404096	13	NULL	NULL	0	NULL	thermoneutral temperature	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On one occasion , exercise was preceded by whole-body cooling achieved by immersion in water during a reduction in temperature from 29 to 24 degrees C , and , for the other trial , by immersion in water at a thermoneutral temperature ( control , 34.8 degrees C ) .
	manualset3
121265	13	404096	13	NULL	NULL	0	NULL	34.8 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On one occasion , exercise was preceded by whole-body cooling achieved by immersion in water during a reduction in temperature from 29 to 24 degrees C , and , for the other trial , by immersion in water at a thermoneutral temperature ( control , 34.8 degrees C ) .
	manualset3
121266	1	404097	13	NULL	NULL	0	NULL	gene-based analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	On optimal gene-based analysis of genome scans .
	manualset3
121267	2	404097	13	NULL	NULL	0	NULL	genome scans	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	On optimal gene-based analysis of genome scans .
	manualset3
121268	1	404098	13	NULL	NULL	0	NULL	reaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On reaction of the 4OHEN-GSH conjugate with NADPH , 4-OHEN was observed to be regenerated at a rate dependent upon NADPH concentration , indicating that intracellular nonenzymatic and enzymatic regeneration of 4-OHEN accounts for the observed estrogenic activity of 4-OHEN .
	manualset3
121269	2	404098	13	NULL	NULL	0	NULL	4OHEN-GSH conjugate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On reaction of the 4OHEN-GSH conjugate with NADPH , 4-OHEN was observed to be regenerated at a rate dependent upon NADPH concentration , indicating that intracellular nonenzymatic and enzymatic regeneration of 4-OHEN accounts for the observed estrogenic activity of 4-OHEN .
	manualset3
121270	3	404098	13	NULL	NULL	0	NULL	NADPH 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On reaction of the 4OHEN-GSH conjugate with NADPH , 4-OHEN was observed to be regenerated at a rate dependent upon NADPH concentration , indicating that intracellular nonenzymatic and enzymatic regeneration of 4-OHEN accounts for the observed estrogenic activity of 4-OHEN .
	manualset3
121271	4	404098	13	NULL	NULL	0	NULL	 4-OHEN	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On reaction of the 4OHEN-GSH conjugate with NADPH , 4-OHEN was observed to be regenerated at a rate dependent upon NADPH concentration , indicating that intracellular nonenzymatic and enzymatic regeneration of 4-OHEN accounts for the observed estrogenic activity of 4-OHEN .
	manualset3
121272	5	404098	13	NULL	NULL	0	NULL	rate 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On reaction of the 4OHEN-GSH conjugate with NADPH , 4-OHEN was observed to be regenerated at a rate dependent upon NADPH concentration , indicating that intracellular nonenzymatic and enzymatic regeneration of 4-OHEN accounts for the observed estrogenic activity of 4-OHEN .
	manualset3
121273	6	404098	13	NULL	NULL	0	NULL	NADPH concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On reaction of the 4OHEN-GSH conjugate with NADPH , 4-OHEN was observed to be regenerated at a rate dependent upon NADPH concentration , indicating that intracellular nonenzymatic and enzymatic regeneration of 4-OHEN accounts for the observed estrogenic activity of 4-OHEN .
	manualset3
121274	7	404098	13	NULL	NULL	0	NULL	nonenzymatic regeneration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On reaction of the 4OHEN-GSH conjugate with NADPH , 4-OHEN was observed to be regenerated at a rate dependent upon NADPH concentration , indicating that intracellular nonenzymatic and enzymatic regeneration of 4-OHEN accounts for the observed estrogenic activity of 4-OHEN .
	manualset3
121275	8	404098	13	NULL	NULL	0	NULL	enzymatic regeneration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On reaction of the 4OHEN-GSH conjugate with NADPH , 4-OHEN was observed to be regenerated at a rate dependent upon NADPH concentration , indicating that intracellular nonenzymatic and enzymatic regeneration of 4-OHEN accounts for the observed estrogenic activity of 4-OHEN .
	manualset3
121276	9	404098	13	NULL	NULL	0	NULL	4-OHEN	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On reaction of the 4OHEN-GSH conjugate with NADPH , 4-OHEN was observed to be regenerated at a rate dependent upon NADPH concentration , indicating that intracellular nonenzymatic and enzymatic regeneration of 4-OHEN accounts for the observed estrogenic activity of 4-OHEN .
	manualset3
121278	11	404098	13	NULL	NULL	0	NULL	estrogenic activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On reaction of the 4OHEN-GSH conjugate with NADPH , 4-OHEN was observed to be regenerated at a rate dependent upon NADPH concentration , indicating that intracellular nonenzymatic and enzymatic regeneration of 4-OHEN accounts for the observed estrogenic activity of 4-OHEN .
	manualset3
121279	12	404098	13	NULL	NULL	0	NULL	4-OHEN 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On reaction of the 4OHEN-GSH conjugate with NADPH , 4-OHEN was observed to be regenerated at a rate dependent upon NADPH concentration , indicating that intracellular nonenzymatic and enzymatic regeneration of 4-OHEN accounts for the observed estrogenic activity of 4-OHEN .
	manualset3
121280	1	404099	13	NULL	NULL	0	NULL	self-sterility 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On self-sterility and inbreeding effect in tetraploid rye .
	manualset3
121281	2	404099	13	NULL	NULL	0	NULL	inbreeding	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On self-sterility and inbreeding effect in tetraploid rye .
	manualset3
121282	3	404099	13	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On self-sterility and inbreeding effect in tetraploid rye .
	manualset3
121283	4	404099	13	NULL	NULL	0	NULL	tetraploid rye	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On self-sterility and inbreeding effect in tetraploid rye .
	manualset3
121284	1	404100	13	NULL	NULL	0	NULL	10th hospitalization day	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	On the 10th hospitalization day , when 40 mg of prednisolone was administered , cardiopulmonary arrest suddenly occurred , and his laboratory data showed hyponatremia and hyperpotassemia .
	manualset3
121285	2	404100	13	NULL	NULL	0	NULL	40 mg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the 10th hospitalization day , when 40 mg of prednisolone was administered , cardiopulmonary arrest suddenly occurred , and his laboratory data showed hyponatremia and hyperpotassemia .
	manualset3
121286	3	404100	13	NULL	NULL	0	NULL	prednisolone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	On the 10th hospitalization day , when 40 mg of prednisolone was administered , cardiopulmonary arrest suddenly occurred , and his laboratory data showed hyponatremia and hyperpotassemia .
	manualset3
121287	4	404100	13	NULL	NULL	0	NULL	cardiopulmonary arrest	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the 10th hospitalization day , when 40 mg of prednisolone was administered , cardiopulmonary arrest suddenly occurred , and his laboratory data showed hyponatremia and hyperpotassemia .
	manualset3
121288	5	404100	13	NULL	NULL	0	NULL	laboratory data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	On the 10th hospitalization day , when 40 mg of prednisolone was administered , cardiopulmonary arrest suddenly occurred , and his laboratory data showed hyponatremia and hyperpotassemia .
	manualset3
121289	6	404100	13	NULL	NULL	0	NULL	hyponatremia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the 10th hospitalization day , when 40 mg of prednisolone was administered , cardiopulmonary arrest suddenly occurred , and his laboratory data showed hyponatremia and hyperpotassemia .
	manualset3
121290	7	404100	13	NULL	NULL	0	NULL	hyperpotassemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the 10th hospitalization day , when 40 mg of prednisolone was administered , cardiopulmonary arrest suddenly occurred , and his laboratory data showed hyponatremia and hyperpotassemia .
	manualset3
121291	1	404101	13	NULL	NULL	0	NULL	deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A deficiency in placental 11 beta-HSD-II enzyme activity was supposed to be the underlying cause .
	manualset3
121292	2	404101	13	NULL	NULL	0	NULL	placental 11 beta-HSD-II enzyme activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A deficiency in placental 11 beta-HSD-II enzyme activity was supposed to be the underlying cause .
	manualset3
121293	3	404101	13	NULL	NULL	0	NULL	cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A deficiency in placental 11 beta-HSD-II enzyme activity was supposed to be the underlying cause .
	manualset3
121294	1	404102	13	NULL	NULL	0	NULL	Molecular Structure	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the Molecular Structure of Uranium Dicarbide : T-Shape versus Linear Isomers .
	manualset3
121295	2	404102	13	NULL	NULL	0	NULL	Uranium Dicarbide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the Molecular Structure of Uranium Dicarbide : T-Shape versus Linear Isomers .
	manualset3
121296	3	404102	13	NULL	NULL	0	NULL	T-Shape Isomers 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the Molecular Structure of Uranium Dicarbide : T-Shape versus Linear Isomers .
	manualset3
121297	4	404102	13	NULL	NULL	0	NULL	Linear Isomers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the Molecular Structure of Uranium Dicarbide : T-Shape versus Linear Isomers .
	manualset3
121298	1	404103	13	NULL	NULL	0	NULL	basis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of EU directives 89/391/EEC ( to encourage improvements in the safety and health of workers at work ) and 2000/54/EC ( on the protection of workers from risks related to exposure to biological agents at work ) , biological hazards at work have to be assessed and preventive measures have to be introduced in all member states of the EU .
	manualset3
121299	2	404103	13	NULL	NULL	0	NULL	EU directives 89/391/EEC	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of EU directives 89/391/EEC ( to encourage improvements in the safety and health of workers at work ) and 2000/54/EC ( on the protection of workers from risks related to exposure to biological agents at work ) , biological hazards at work have to be assessed and preventive measures have to be introduced in all member states of the EU .
	manualset3
121300	3	404103	13	NULL	NULL	0	NULL	improvements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of EU directives 89/391/EEC ( to encourage improvements in the safety and health of workers at work ) and 2000/54/EC ( on the protection of workers from risks related to exposure to biological agents at work ) , biological hazards at work have to be assessed and preventive measures have to be introduced in all member states of the EU .
	manualset3
121301	4	404103	13	NULL	NULL	0	NULL	safety	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of EU directives 89/391/EEC ( to encourage improvements in the safety and health of workers at work ) and 2000/54/EC ( on the protection of workers from risks related to exposure to biological agents at work ) , biological hazards at work have to be assessed and preventive measures have to be introduced in all member states of the EU .
	manualset3
121302	5	404103	13	NULL	NULL	0	NULL	health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of EU directives 89/391/EEC ( to encourage improvements in the safety and health of workers at work ) and 2000/54/EC ( on the protection of workers from risks related to exposure to biological agents at work ) , biological hazards at work have to be assessed and preventive measures have to be introduced in all member states of the EU .
	manualset3
121303	6	404103	13	NULL	NULL	0	NULL	workers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of EU directives 89/391/EEC ( to encourage improvements in the safety and health of workers at work ) and 2000/54/EC ( on the protection of workers from risks related to exposure to biological agents at work ) , biological hazards at work have to be assessed and preventive measures have to be introduced in all member states of the EU .
	manualset3
121304	7	404103	13	NULL	NULL	0	NULL	work 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of EU directives 89/391/EEC ( to encourage improvements in the safety and health of workers at work ) and 2000/54/EC ( on the protection of workers from risks related to exposure to biological agents at work ) , biological hazards at work have to be assessed and preventive measures have to be introduced in all member states of the EU .
	manualset3
121305	8	404103	13	NULL	NULL	0	NULL	2000/54/EC 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of EU directives 89/391/EEC ( to encourage improvements in the safety and health of workers at work ) and 2000/54/EC ( on the protection of workers from risks related to exposure to biological agents at work ) , biological hazards at work have to be assessed and preventive measures have to be introduced in all member states of the EU .
	manualset3
121306	9	404103	13	NULL	NULL	0	NULL	protection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of EU directives 89/391/EEC ( to encourage improvements in the safety and health of workers at work ) and 2000/54/EC ( on the protection of workers from risks related to exposure to biological agents at work ) , biological hazards at work have to be assessed and preventive measures have to be introduced in all member states of the EU .
	manualset3
121307	10	404103	13	NULL	NULL	0	NULL	workers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of EU directives 89/391/EEC ( to encourage improvements in the safety and health of workers at work ) and 2000/54/EC ( on the protection of workers from risks related to exposure to biological agents at work ) , biological hazards at work have to be assessed and preventive measures have to be introduced in all member states of the EU .
	manualset3
121310	11	404103	13	NULL	NULL	0	NULL	risks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of EU directives 89/391/EEC ( to encourage improvements in the safety and health of workers at work ) and 2000/54/EC ( on the protection of workers from risks related to exposure to biological agents at work ) , biological hazards at work have to be assessed and preventive measures have to be introduced in all member states of the EU .
	manualset3
121311	12	404103	13	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of EU directives 89/391/EEC ( to encourage improvements in the safety and health of workers at work ) and 2000/54/EC ( on the protection of workers from risks related to exposure to biological agents at work ) , biological hazards at work have to be assessed and preventive measures have to be introduced in all member states of the EU .
	manualset3
121312	13	404103	13	NULL	NULL	0	NULL	biological agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of EU directives 89/391/EEC ( to encourage improvements in the safety and health of workers at work ) and 2000/54/EC ( on the protection of workers from risks related to exposure to biological agents at work ) , biological hazards at work have to be assessed and preventive measures have to be introduced in all member states of the EU .
	manualset3
121313	14	404103	13	NULL	NULL	0	NULL	work	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of EU directives 89/391/EEC ( to encourage improvements in the safety and health of workers at work ) and 2000/54/EC ( on the protection of workers from risks related to exposure to biological agents at work ) , biological hazards at work have to be assessed and preventive measures have to be introduced in all member states of the EU .
	manualset3
121314	15	404103	13	NULL	NULL	0	NULL	biological hazards	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of EU directives 89/391/EEC ( to encourage improvements in the safety and health of workers at work ) and 2000/54/EC ( on the protection of workers from risks related to exposure to biological agents at work ) , biological hazards at work have to be assessed and preventive measures have to be introduced in all member states of the EU .
	manualset3
121315	16	404103	13	NULL	NULL	0	NULL	work 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of EU directives 89/391/EEC ( to encourage improvements in the safety and health of workers at work ) and 2000/54/EC ( on the protection of workers from risks related to exposure to biological agents at work ) , biological hazards at work have to be assessed and preventive measures have to be introduced in all member states of the EU .
	manualset3
121316	17	404103	13	NULL	NULL	0	NULL	preventive measures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of EU directives 89/391/EEC ( to encourage improvements in the safety and health of workers at work ) and 2000/54/EC ( on the protection of workers from risks related to exposure to biological agents at work ) , biological hazards at work have to be assessed and preventive measures have to be introduced in all member states of the EU .
	manualset3
121317	18	404103	13	NULL	NULL	0	NULL	member states	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of EU directives 89/391/EEC ( to encourage improvements in the safety and health of workers at work ) and 2000/54/EC ( on the protection of workers from risks related to exposure to biological agents at work ) , biological hazards at work have to be assessed and preventive measures have to be introduced in all member states of the EU .
	manualset3
121318	19	404103	13	NULL	NULL	0	NULL	EU	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of EU directives 89/391/EEC ( to encourage improvements in the safety and health of workers at work ) and 2000/54/EC ( on the protection of workers from risks related to exposure to biological agents at work ) , biological hazards at work have to be assessed and preventive measures have to be introduced in all member states of the EU .
	manualset3
121320	1	404104	13	NULL	NULL	0	NULL	basis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of VP4 sequence analysis , a potential distinct subgroup within HRV-C has also been identified , although more complete genome sequences are needed to better define the genetic diversity of HRV-C .
	manualset3
121322	2	404104	13	NULL	NULL	0	NULL	VP4 sequence analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of VP4 sequence analysis , a potential distinct subgroup within HRV-C has also been identified , although more complete genome sequences are needed to better define the genetic diversity of HRV-C .
	manualset3
121333	3	404104	13	NULL	NULL	0	NULL	subgroup 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of VP4 sequence analysis , a potential distinct subgroup within HRV-C has also been identified , although more complete genome sequences are needed to better define the genetic diversity of HRV-C .
	manualset3
121334	4	404104	13	NULL	NULL	0	NULL	HRV-C	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of VP4 sequence analysis , a potential distinct subgroup within HRV-C has also been identified , although more complete genome sequences are needed to better define the genetic diversity of HRV-C .
	manualset3
121335	5	404104	13	NULL	NULL	0	NULL	genome sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of VP4 sequence analysis , a potential distinct subgroup within HRV-C has also been identified , although more complete genome sequences are needed to better define the genetic diversity of HRV-C .
	manualset3
121336	6	404104	13	NULL	NULL	0	NULL	genetic diversity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of VP4 sequence analysis , a potential distinct subgroup within HRV-C has also been identified , although more complete genome sequences are needed to better define the genetic diversity of HRV-C .
	manualset3
121337	7	404104	13	NULL	NULL	0	NULL	HRV-C	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of VP4 sequence analysis , a potential distinct subgroup within HRV-C has also been identified , although more complete genome sequences are needed to better define the genetic diversity of HRV-C .
	manualset3
121338	1	404105	13	NULL	NULL	0	NULL	basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of a two-compartment model we interpreted our findings by assuming an unequal distribution of diffusion and convective O ( 2 ) transport in the pulmonary gas exchange of the patients .
	manualset3
121339	2	404105	13	NULL	NULL	NULL	NULL	two-compartment model	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On the basis of a two-compartment model we interpreted our findings by assuming an unequal distribution of diffusion and convective O ( 2 ) transport in the pulmonary gas exchange of the patients .
	manualset3
121340	3	404105	13	NULL	NULL	NULL	NULL	findings	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On the basis of a two-compartment model we interpreted our findings by assuming an unequal distribution of diffusion and convective O ( 2 ) transport in the pulmonary gas exchange of the patients .
	manualset3
121341	4	404105	13	NULL	NULL	0	NULL	distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of a two-compartment model we interpreted our findings by assuming an unequal distribution of diffusion and convective O ( 2 ) transport in the pulmonary gas exchange of the patients .
	manualset3
121342	5	404105	13	NULL	NULL	0	NULL	diffusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of a two-compartment model we interpreted our findings by assuming an unequal distribution of diffusion and convective O ( 2 ) transport in the pulmonary gas exchange of the patients .
	manualset3
121343	6	404105	13	NULL	NULL	0	NULL	convective O ( 2 ) transport	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of a two-compartment model we interpreted our findings by assuming an unequal distribution of diffusion and convective O ( 2 ) transport in the pulmonary gas exchange of the patients .
	manualset3
121344	7	404105	13	NULL	NULL	0	NULL	pulmonary gas exchange 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of a two-compartment model we interpreted our findings by assuming an unequal distribution of diffusion and convective O ( 2 ) transport in the pulmonary gas exchange of the patients .
	manualset3
121345	8	404105	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of a two-compartment model we interpreted our findings by assuming an unequal distribution of diffusion and convective O ( 2 ) transport in the pulmonary gas exchange of the patients .
	manualset3
121346	1	404106	13	NULL	NULL	0	NULL	basis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of colocalisation of neurochemical markers and knowledge gained from previous studies of neural projections , 17 classes of neurons were identified .
	manualset3
121347	2	404106	13	NULL	NULL	0	NULL	colocalisation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of colocalisation of neurochemical markers and knowledge gained from previous studies of neural projections , 17 classes of neurons were identified .
	manualset3
121348	3	404106	13	NULL	NULL	0	NULL	neurochemical markers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of colocalisation of neurochemical markers and knowledge gained from previous studies of neural projections , 17 classes of neurons were identified .
	manualset3
121349	4	404106	13	NULL	NULL	0	NULL	knowledge 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of colocalisation of neurochemical markers and knowledge gained from previous studies of neural projections , 17 classes of neurons were identified .
	manualset3
121350	5	404106	13	NULL	NULL	0	NULL	previous studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of colocalisation of neurochemical markers and knowledge gained from previous studies of neural projections , 17 classes of neurons were identified .
	manualset3
121351	6	404106	13	NULL	NULL	0	NULL	neural projections	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of colocalisation of neurochemical markers and knowledge gained from previous studies of neural projections , 17 classes of neurons were identified .
	manualset3
121352	7	404106	13	NULL	NULL	0	NULL	17 classes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of colocalisation of neurochemical markers and knowledge gained from previous studies of neural projections , 17 classes of neurons were identified .
	manualset3
121353	8	404106	13	NULL	NULL	0	NULL	neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of colocalisation of neurochemical markers and knowledge gained from previous studies of neural projections , 17 classes of neurons were identified .
	manualset3
121354	1	404107	13	NULL	NULL	0	NULL	basis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of established practice guidelines , liposomal amphotericin B ( L-AMB ) was administered to avoid the possible nephrotoxicity of amphotericin B. After the treatment was started , the patient 's condition gradually improved .
	manualset3
121355	2	404107	13	NULL	NULL	0	NULL	practice guidelines 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of established practice guidelines , liposomal amphotericin B ( L-AMB ) was administered to avoid the possible nephrotoxicity of amphotericin B. After the treatment was started , the patient 's condition gradually improved .
	manualset3
121356	3	404107	13	NULL	NULL	0	NULL	liposomal amphotericin B ( L-AMB )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of established practice guidelines , liposomal amphotericin B ( L-AMB ) was administered to avoid the possible nephrotoxicity of amphotericin B. After the treatment was started , the patient 's condition gradually improved .
	manualset3
121357	4	404107	13	NULL	NULL	0	NULL	nephrotoxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of established practice guidelines , liposomal amphotericin B ( L-AMB ) was administered to avoid the possible nephrotoxicity of amphotericin B. After the treatment was started , the patient 's condition gradually improved .
	manualset3
121358	5	404107	13	NULL	NULL	0	NULL	amphotericin B	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of established practice guidelines , liposomal amphotericin B ( L-AMB ) was administered to avoid the possible nephrotoxicity of amphotericin B. After the treatment was started , the patient 's condition gradually improved .
	manualset3
121359	6	404107	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of established practice guidelines , liposomal amphotericin B ( L-AMB ) was administered to avoid the possible nephrotoxicity of amphotericin B. After the treatment was started , the patient 's condition gradually improved .
	manualset3
121360	7	404107	13	NULL	NULL	0	NULL	patient 's 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of established practice guidelines , liposomal amphotericin B ( L-AMB ) was administered to avoid the possible nephrotoxicity of amphotericin B. After the treatment was started , the patient 's condition gradually improved .
	manualset3
121361	1	404108	13	NULL	NULL	0	NULL	basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of graphical and statistical comparison of the pharmacokinetic parameters ( AUC0-infinity , AUCss , 0-tau , tmax , Cmax , Css , min , Css , av , MRT , etc. ) calculated from the time-plasma concentration curve , moreover on the basis of clinical results , there was no significant difference between the two preparations .
	manualset3
121362	2	404108	13	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of graphical and statistical comparison of the pharmacokinetic parameters ( AUC0-infinity , AUCss , 0-tau , tmax , Cmax , Css , min , Css , av , MRT , etc. ) calculated from the time-plasma concentration curve , moreover on the basis of clinical results , there was no significant difference between the two preparations .
	manualset3
121363	3	404108	13	NULL	NULL	0	NULL	pharmacokinetic parameters	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of graphical and statistical comparison of the pharmacokinetic parameters ( AUC0-infinity , AUCss , 0-tau , tmax , Cmax , Css , min , Css , av , MRT , etc. ) calculated from the time-plasma concentration curve , moreover on the basis of clinical results , there was no significant difference between the two preparations .
	manualset3
121364	4	404108	13	NULL	NULL	0	NULL	AUC0-infinity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of graphical and statistical comparison of the pharmacokinetic parameters ( AUC0-infinity , AUCss , 0-tau , tmax , Cmax , Css , min , Css , av , MRT , etc. ) calculated from the time-plasma concentration curve , moreover on the basis of clinical results , there was no significant difference between the two preparations .
	manualset3
121365	5	404108	13	NULL	NULL	0	NULL	AUCss	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of graphical and statistical comparison of the pharmacokinetic parameters ( AUC0-infinity , AUCss , 0-tau , tmax , Cmax , Css , min , Css , av , MRT , etc. ) calculated from the time-plasma concentration curve , moreover on the basis of clinical results , there was no significant difference between the two preparations .
	manualset3
121366	6	404108	13	NULL	NULL	0	NULL	0-tau	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of graphical and statistical comparison of the pharmacokinetic parameters ( AUC0-infinity , AUCss , 0-tau , tmax , Cmax , Css , min , Css , av , MRT , etc. ) calculated from the time-plasma concentration curve , moreover on the basis of clinical results , there was no significant difference between the two preparations .
	manualset3
121367	7	404108	13	NULL	NULL	0	NULL	tmax	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of graphical and statistical comparison of the pharmacokinetic parameters ( AUC0-infinity , AUCss , 0-tau , tmax , Cmax , Css , min , Css , av , MRT , etc. ) calculated from the time-plasma concentration curve , moreover on the basis of clinical results , there was no significant difference between the two preparations .
	manualset3
121368	8	404108	13	NULL	NULL	0	NULL	Cmax	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of graphical and statistical comparison of the pharmacokinetic parameters ( AUC0-infinity , AUCss , 0-tau , tmax , Cmax , Css , min , Css , av , MRT , etc. ) calculated from the time-plasma concentration curve , moreover on the basis of clinical results , there was no significant difference between the two preparations .
	manualset3
121369	9	404108	13	NULL	NULL	0	NULL	Css	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of graphical and statistical comparison of the pharmacokinetic parameters ( AUC0-infinity , AUCss , 0-tau , tmax , Cmax , Css , min , Css , av , MRT , etc. ) calculated from the time-plasma concentration curve , moreover on the basis of clinical results , there was no significant difference between the two preparations .
	manualset3
121370	10	404108	13	NULL	NULL	0	NULL	min	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of graphical and statistical comparison of the pharmacokinetic parameters ( AUC0-infinity , AUCss , 0-tau , tmax , Cmax , Css , min , Css , av , MRT , etc. ) calculated from the time-plasma concentration curve , moreover on the basis of clinical results , there was no significant difference between the two preparations .
	manualset3
121371	11	404108	13	NULL	NULL	0	NULL	Css	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of graphical and statistical comparison of the pharmacokinetic parameters ( AUC0-infinity , AUCss , 0-tau , tmax , Cmax , Css , min , Css , av , MRT , etc. ) calculated from the time-plasma concentration curve , moreover on the basis of clinical results , there was no significant difference between the two preparations .
	manualset3
121372	12	404108	13	NULL	NULL	0	NULL	av	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of graphical and statistical comparison of the pharmacokinetic parameters ( AUC0-infinity , AUCss , 0-tau , tmax , Cmax , Css , min , Css , av , MRT , etc. ) calculated from the time-plasma concentration curve , moreover on the basis of clinical results , there was no significant difference between the two preparations .
	manualset3
121373	13	404108	13	NULL	NULL	0	NULL	MRT	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of graphical and statistical comparison of the pharmacokinetic parameters ( AUC0-infinity , AUCss , 0-tau , tmax , Cmax , Css , min , Css , av , MRT , etc. ) calculated from the time-plasma concentration curve , moreover on the basis of clinical results , there was no significant difference between the two preparations .
	manualset3
121374	14	404108	13	NULL	NULL	0	NULL	 time-plasma concentration curve	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of graphical and statistical comparison of the pharmacokinetic parameters ( AUC0-infinity , AUCss , 0-tau , tmax , Cmax , Css , min , Css , av , MRT , etc. ) calculated from the time-plasma concentration curve , moreover on the basis of clinical results , there was no significant difference between the two preparations .
	manualset3
121375	15	404108	13	NULL	NULL	0	NULL	basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of graphical and statistical comparison of the pharmacokinetic parameters ( AUC0-infinity , AUCss , 0-tau , tmax , Cmax , Css , min , Css , av , MRT , etc. ) calculated from the time-plasma concentration curve , moreover on the basis of clinical results , there was no significant difference between the two preparations .
	manualset3
121376	16	404108	13	NULL	NULL	0	NULL	clinical results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of graphical and statistical comparison of the pharmacokinetic parameters ( AUC0-infinity , AUCss , 0-tau , tmax , Cmax , Css , min , Css , av , MRT , etc. ) calculated from the time-plasma concentration curve , moreover on the basis of clinical results , there was no significant difference between the two preparations .
	manualset3
121377	17	404108	13	NULL	NULL	0	NULL	difference 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of graphical and statistical comparison of the pharmacokinetic parameters ( AUC0-infinity , AUCss , 0-tau , tmax , Cmax , Css , min , Css , av , MRT , etc. ) calculated from the time-plasma concentration curve , moreover on the basis of clinical results , there was no significant difference between the two preparations .
	manualset3
121378	18	404108	13	NULL	NULL	NULL	NULL	preparations	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On the basis of graphical and statistical comparison of the pharmacokinetic parameters ( AUC0-infinity , AUCss , 0-tau , tmax , Cmax , Css , min , Css , av , MRT , etc. ) calculated from the time-plasma concentration curve , moreover on the basis of clinical results , there was no significant difference between the two preparations .
	manualset3
121379	1	404109	13	NULL	NULL	0	NULL	maximum	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A definite maximum of snake bites was observed during October and November which corresponds to the transition from rainy to dry season .
	manualset3
121380	2	404109	13	NULL	NULL	0	NULL	snake bites	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A definite maximum of snake bites was observed during October and November which corresponds to the transition from rainy to dry season .
	manualset3
121381	3	404109	13	NULL	NULL	0	NULL	October 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	A definite maximum of snake bites was observed during October and November which corresponds to the transition from rainy to dry season .
	manualset3
121382	4	404109	13	NULL	NULL	0	NULL	November 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	A definite maximum of snake bites was observed during October and November which corresponds to the transition from rainy to dry season .
	manualset3
121383	5	404109	13	NULL	NULL	0	NULL	transition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A definite maximum of snake bites was observed during October and November which corresponds to the transition from rainy to dry season .
	manualset3
121384	6	404109	13	NULL	NULL	0	NULL	rainy season	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A definite maximum of snake bites was observed during October and November which corresponds to the transition from rainy to dry season .
	manualset3
121385	7	404109	13	NULL	NULL	0	NULL	dry season	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A definite maximum of snake bites was observed during October and November which corresponds to the transition from rainy to dry season .
	manualset3
121386	1	404110	13	NULL	NULL	0	NULL	basis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of our results , combined with that of others , we suggest that in Csb the transcriptional response predominates during early development , whereas a neurodegenerative response associated with repair deficits predominates in later life .
	manualset3
121387	2	404110	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of our results , combined with that of others , we suggest that in Csb the transcriptional response predominates during early development , whereas a neurodegenerative response associated with repair deficits predominates in later life .
	manualset3
121388	3	404110	13	NULL	NULL	NULL	NULL	Csb	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On the basis of our results , combined with that of others , we suggest that in Csb the transcriptional response predominates during early development , whereas a neurodegenerative response associated with repair deficits predominates in later life .
	manualset3
121389	4	404110	13	NULL	NULL	0	NULL	transcriptional response 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of our results , combined with that of others , we suggest that in Csb the transcriptional response predominates during early development , whereas a neurodegenerative response associated with repair deficits predominates in later life .
	manualset3
121390	5	404110	13	NULL	NULL	0	NULL	development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of our results , combined with that of others , we suggest that in Csb the transcriptional response predominates during early development , whereas a neurodegenerative response associated with repair deficits predominates in later life .
	manualset3
121391	6	404110	13	NULL	NULL	0	NULL	neurodegenerative response 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of our results , combined with that of others , we suggest that in Csb the transcriptional response predominates during early development , whereas a neurodegenerative response associated with repair deficits predominates in later life .
	manualset3
121392	7	404110	13	NULL	NULL	0	NULL	repair deficits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of our results , combined with that of others , we suggest that in Csb the transcriptional response predominates during early development , whereas a neurodegenerative response associated with repair deficits predominates in later life .
	manualset3
121393	8	404110	13	NULL	NULL	0	NULL	later life	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of our results , combined with that of others , we suggest that in Csb the transcriptional response predominates during early development , whereas a neurodegenerative response associated with repair deficits predominates in later life .
	manualset3
121394	1	404111	13	NULL	NULL	0	NULL	basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of our results , the importance of eosinophilic granular cells in a decidualization process is hypothesized to occur also in the bitch .
	manualset3
121395	2	404111	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of our results , the importance of eosinophilic granular cells in a decidualization process is hypothesized to occur also in the bitch .
	manualset3
121396	3	404111	13	NULL	NULL	0	NULL	importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of our results , the importance of eosinophilic granular cells in a decidualization process is hypothesized to occur also in the bitch .
	manualset3
121397	4	404111	13	NULL	NULL	0	NULL	eosinophilic granular cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of our results , the importance of eosinophilic granular cells in a decidualization process is hypothesized to occur also in the bitch .
	manualset3
121398	5	404111	13	NULL	NULL	0	NULL	decidualization process	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of our results , the importance of eosinophilic granular cells in a decidualization process is hypothesized to occur also in the bitch .
	manualset3
121399	6	404111	13	NULL	NULL	0	NULL	bitch	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of our results , the importance of eosinophilic granular cells in a decidualization process is hypothesized to occur also in the bitch .
	manualset3
121400	1	404112	13	NULL	NULL	0	NULL	basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of synthesized negatively charged hydrosol hexacianferrate ( II ) ferrum ( III ) ( HCFF ) by diameter 10-20 HM are received stable conjugates with antibodies and antigens glycoprotein and lipopolysaccharide ( LPS ) nature .
	manualset3
121401	2	404112	13	NULL	NULL	0	NULL	hydrosol hexacianferrate ( II ) ferrum ( III ) ( HCFF )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of synthesized negatively charged hydrosol hexacianferrate ( II ) ferrum ( III ) ( HCFF ) by diameter 10-20 HM are received stable conjugates with antibodies and antigens glycoprotein and lipopolysaccharide ( LPS ) nature .
	manualset3
121402	3	404112	13	NULL	NULL	0	NULL	diameter 10-20 HM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of synthesized negatively charged hydrosol hexacianferrate ( II ) ferrum ( III ) ( HCFF ) by diameter 10-20 HM are received stable conjugates with antibodies and antigens glycoprotein and lipopolysaccharide ( LPS ) nature .
	manualset3
121403	4	404112	13	NULL	NULL	0	NULL	conjugates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of synthesized negatively charged hydrosol hexacianferrate ( II ) ferrum ( III ) ( HCFF ) by diameter 10-20 HM are received stable conjugates with antibodies and antigens glycoprotein and lipopolysaccharide ( LPS ) nature .
	manualset3
121404	5	404112	13	NULL	NULL	0	NULL	antibodies 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of synthesized negatively charged hydrosol hexacianferrate ( II ) ferrum ( III ) ( HCFF ) by diameter 10-20 HM are received stable conjugates with antibodies and antigens glycoprotein and lipopolysaccharide ( LPS ) nature .
	manualset3
121405	6	404112	13	NULL	NULL	NULL	NULL	glycoprotein nature 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On the basis of synthesized negatively charged hydrosol hexacianferrate ( II ) ferrum ( III ) ( HCFF ) by diameter 10-20 HM are received stable conjugates with antibodies and antigens glycoprotein and lipopolysaccharide ( LPS ) nature .
	manualset3
121406	7	404112	13	NULL	NULL	0	NULL	lipopolysaccharide ( LPS ) nature 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of synthesized negatively charged hydrosol hexacianferrate ( II ) ferrum ( III ) ( HCFF ) by diameter 10-20 HM are received stable conjugates with antibodies and antigens glycoprotein and lipopolysaccharide ( LPS ) nature .
	manualset3
121407	8	404112	13	NULL	NULL	0	NULL	antigens 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of synthesized negatively charged hydrosol hexacianferrate ( II ) ferrum ( III ) ( HCFF ) by diameter 10-20 HM are received stable conjugates with antibodies and antigens glycoprotein and lipopolysaccharide ( LPS ) nature .
	manualset3
121408	1	404113	13	NULL	NULL	0	NULL	basis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the German Transplant Law guidelines for `` Requirements regarding quality control for procedures related to organ procurement and transplantation '' have been formulated by the German Medical Chamber .
	manualset3
121409	2	404113	13	NULL	NULL	0	NULL	German Transplant Law guidelines	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the German Transplant Law guidelines for `` Requirements regarding quality control for procedures related to organ procurement and transplantation '' have been formulated by the German Medical Chamber .
	manualset3
121410	3	404113	13	NULL	NULL	NULL	NULL	Requirements 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On the basis of the German Transplant Law guidelines for `` Requirements regarding quality control for procedures related to organ procurement and transplantation '' have been formulated by the German Medical Chamber .
	manualset3
121411	4	404113	13	NULL	NULL	0	NULL	quality control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the German Transplant Law guidelines for `` Requirements regarding quality control for procedures related to organ procurement and transplantation '' have been formulated by the German Medical Chamber .
	manualset3
121412	5	404113	13	NULL	NULL	0	NULL	procedures 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the German Transplant Law guidelines for `` Requirements regarding quality control for procedures related to organ procurement and transplantation '' have been formulated by the German Medical Chamber .
	manualset3
121413	6	404113	13	NULL	NULL	0	NULL	organ procurement	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the German Transplant Law guidelines for `` Requirements regarding quality control for procedures related to organ procurement and transplantation '' have been formulated by the German Medical Chamber .
	manualset3
121414	7	404113	13	NULL	NULL	0	NULL	transplantation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the German Transplant Law guidelines for `` Requirements regarding quality control for procedures related to organ procurement and transplantation '' have been formulated by the German Medical Chamber .
	manualset3
121415	8	404113	13	NULL	NULL	0	NULL	German Medical Chamber	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the German Transplant Law guidelines for `` Requirements regarding quality control for procedures related to organ procurement and transplantation '' have been formulated by the German Medical Chamber .
	manualset3
121416	1	404114	13	NULL	NULL	0	NULL	basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the comparison of electron-transfer reactions in the two enzymes , we conclude that the transfer rate of the fourth electron to the binuclear center is not only determined by the electron-transfer rate from haem a to the binuclear center , but also by the electron equilibrium between CuA and haem a. In addition , in contrast to the bovine enzyme , where the electron - and proton-transfer rates during oxidation of the fully reduced enzyme by O2 are all faster than the overall turnover rate , in the R. sphaeroides enzyme , the slowest kinetic phase was rate limiting for the overall turnover .
	manualset3
121417	2	404114	13	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the comparison of electron-transfer reactions in the two enzymes , we conclude that the transfer rate of the fourth electron to the binuclear center is not only determined by the electron-transfer rate from haem a to the binuclear center , but also by the electron equilibrium between CuA and haem a. In addition , in contrast to the bovine enzyme , where the electron - and proton-transfer rates during oxidation of the fully reduced enzyme by O2 are all faster than the overall turnover rate , in the R. sphaeroides enzyme , the slowest kinetic phase was rate limiting for the overall turnover .
	manualset3
121418	3	404114	13	NULL	NULL	0	NULL	electron-transfer reactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the comparison of electron-transfer reactions in the two enzymes , we conclude that the transfer rate of the fourth electron to the binuclear center is not only determined by the electron-transfer rate from haem a to the binuclear center , but also by the electron equilibrium between CuA and haem a. In addition , in contrast to the bovine enzyme , where the electron - and proton-transfer rates during oxidation of the fully reduced enzyme by O2 are all faster than the overall turnover rate , in the R. sphaeroides enzyme , the slowest kinetic phase was rate limiting for the overall turnover .
	manualset3
121419	4	404114	13	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the comparison of electron-transfer reactions in the two enzymes , we conclude that the transfer rate of the fourth electron to the binuclear center is not only determined by the electron-transfer rate from haem a to the binuclear center , but also by the electron equilibrium between CuA and haem a. In addition , in contrast to the bovine enzyme , where the electron - and proton-transfer rates during oxidation of the fully reduced enzyme by O2 are all faster than the overall turnover rate , in the R. sphaeroides enzyme , the slowest kinetic phase was rate limiting for the overall turnover .
	manualset3
121420	5	404114	13	NULL	NULL	0	NULL	enzymes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the comparison of electron-transfer reactions in the two enzymes , we conclude that the transfer rate of the fourth electron to the binuclear center is not only determined by the electron-transfer rate from haem a to the binuclear center , but also by the electron equilibrium between CuA and haem a. In addition , in contrast to the bovine enzyme , where the electron - and proton-transfer rates during oxidation of the fully reduced enzyme by O2 are all faster than the overall turnover rate , in the R. sphaeroides enzyme , the slowest kinetic phase was rate limiting for the overall turnover .
	manualset3
121421	6	404114	13	NULL	NULL	0	NULL	transfer rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the comparison of electron-transfer reactions in the two enzymes , we conclude that the transfer rate of the fourth electron to the binuclear center is not only determined by the electron-transfer rate from haem a to the binuclear center , but also by the electron equilibrium between CuA and haem a. In addition , in contrast to the bovine enzyme , where the electron - and proton-transfer rates during oxidation of the fully reduced enzyme by O2 are all faster than the overall turnover rate , in the R. sphaeroides enzyme , the slowest kinetic phase was rate limiting for the overall turnover .
	manualset3
121422	7	404114	13	NULL	NULL	0	NULL	fourth electron	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the comparison of electron-transfer reactions in the two enzymes , we conclude that the transfer rate of the fourth electron to the binuclear center is not only determined by the electron-transfer rate from haem a to the binuclear center , but also by the electron equilibrium between CuA and haem a. In addition , in contrast to the bovine enzyme , where the electron - and proton-transfer rates during oxidation of the fully reduced enzyme by O2 are all faster than the overall turnover rate , in the R. sphaeroides enzyme , the slowest kinetic phase was rate limiting for the overall turnover .
	manualset3
121423	8	404114	13	NULL	NULL	0	NULL	binuclear center	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the comparison of electron-transfer reactions in the two enzymes , we conclude that the transfer rate of the fourth electron to the binuclear center is not only determined by the electron-transfer rate from haem a to the binuclear center , but also by the electron equilibrium between CuA and haem a. In addition , in contrast to the bovine enzyme , where the electron - and proton-transfer rates during oxidation of the fully reduced enzyme by O2 are all faster than the overall turnover rate , in the R. sphaeroides enzyme , the slowest kinetic phase was rate limiting for the overall turnover .
	manualset3
121424	9	404114	13	NULL	NULL	0	NULL	electron-transfer rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the comparison of electron-transfer reactions in the two enzymes , we conclude that the transfer rate of the fourth electron to the binuclear center is not only determined by the electron-transfer rate from haem a to the binuclear center , but also by the electron equilibrium between CuA and haem a. In addition , in contrast to the bovine enzyme , where the electron - and proton-transfer rates during oxidation of the fully reduced enzyme by O2 are all faster than the overall turnover rate , in the R. sphaeroides enzyme , the slowest kinetic phase was rate limiting for the overall turnover .
	manualset3
121425	10	404114	13	NULL	NULL	NULL	NULL	haem a	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On the basis of the comparison of electron-transfer reactions in the two enzymes , we conclude that the transfer rate of the fourth electron to the binuclear center is not only determined by the electron-transfer rate from haem a to the binuclear center , but also by the electron equilibrium between CuA and haem a. In addition , in contrast to the bovine enzyme , where the electron - and proton-transfer rates during oxidation of the fully reduced enzyme by O2 are all faster than the overall turnover rate , in the R. sphaeroides enzyme , the slowest kinetic phase was rate limiting for the overall turnover .
	manualset3
121426	11	404114	13	NULL	NULL	0	NULL	binuclear center	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the comparison of electron-transfer reactions in the two enzymes , we conclude that the transfer rate of the fourth electron to the binuclear center is not only determined by the electron-transfer rate from haem a to the binuclear center , but also by the electron equilibrium between CuA and haem a. In addition , in contrast to the bovine enzyme , where the electron - and proton-transfer rates during oxidation of the fully reduced enzyme by O2 are all faster than the overall turnover rate , in the R. sphaeroides enzyme , the slowest kinetic phase was rate limiting for the overall turnover .
	manualset3
121427	12	404114	13	NULL	NULL	0	NULL	electron equilibrium	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the comparison of electron-transfer reactions in the two enzymes , we conclude that the transfer rate of the fourth electron to the binuclear center is not only determined by the electron-transfer rate from haem a to the binuclear center , but also by the electron equilibrium between CuA and haem a. In addition , in contrast to the bovine enzyme , where the electron - and proton-transfer rates during oxidation of the fully reduced enzyme by O2 are all faster than the overall turnover rate , in the R. sphaeroides enzyme , the slowest kinetic phase was rate limiting for the overall turnover .
	manualset3
121428	13	404114	13	NULL	NULL	0	NULL	CuA 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the comparison of electron-transfer reactions in the two enzymes , we conclude that the transfer rate of the fourth electron to the binuclear center is not only determined by the electron-transfer rate from haem a to the binuclear center , but also by the electron equilibrium between CuA and haem a. In addition , in contrast to the bovine enzyme , where the electron - and proton-transfer rates during oxidation of the fully reduced enzyme by O2 are all faster than the overall turnover rate , in the R. sphaeroides enzyme , the slowest kinetic phase was rate limiting for the overall turnover .
	manualset3
121429	14	404114	13	NULL	NULL	NULL	NULL	haem a	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On the basis of the comparison of electron-transfer reactions in the two enzymes , we conclude that the transfer rate of the fourth electron to the binuclear center is not only determined by the electron-transfer rate from haem a to the binuclear center , but also by the electron equilibrium between CuA and haem a. In addition , in contrast to the bovine enzyme , where the electron - and proton-transfer rates during oxidation of the fully reduced enzyme by O2 are all faster than the overall turnover rate , in the R. sphaeroides enzyme , the slowest kinetic phase was rate limiting for the overall turnover .
	manualset3
121430	15	404114	13	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the comparison of electron-transfer reactions in the two enzymes , we conclude that the transfer rate of the fourth electron to the binuclear center is not only determined by the electron-transfer rate from haem a to the binuclear center , but also by the electron equilibrium between CuA and haem a. In addition , in contrast to the bovine enzyme , where the electron - and proton-transfer rates during oxidation of the fully reduced enzyme by O2 are all faster than the overall turnover rate , in the R. sphaeroides enzyme , the slowest kinetic phase was rate limiting for the overall turnover .
	manualset3
121431	16	404114	13	NULL	NULL	0	NULL	bovine enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the comparison of electron-transfer reactions in the two enzymes , we conclude that the transfer rate of the fourth electron to the binuclear center is not only determined by the electron-transfer rate from haem a to the binuclear center , but also by the electron equilibrium between CuA and haem a. In addition , in contrast to the bovine enzyme , where the electron - and proton-transfer rates during oxidation of the fully reduced enzyme by O2 are all faster than the overall turnover rate , in the R. sphaeroides enzyme , the slowest kinetic phase was rate limiting for the overall turnover .
	manualset3
121432	17	404114	13	NULL	NULL	0	NULL	electron -transfer rates	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the comparison of electron-transfer reactions in the two enzymes , we conclude that the transfer rate of the fourth electron to the binuclear center is not only determined by the electron-transfer rate from haem a to the binuclear center , but also by the electron equilibrium between CuA and haem a. In addition , in contrast to the bovine enzyme , where the electron - and proton-transfer rates during oxidation of the fully reduced enzyme by O2 are all faster than the overall turnover rate , in the R. sphaeroides enzyme , the slowest kinetic phase was rate limiting for the overall turnover .
	manualset3
121433	18	404114	13	NULL	NULL	0	NULL	proton-transfer rates	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the comparison of electron-transfer reactions in the two enzymes , we conclude that the transfer rate of the fourth electron to the binuclear center is not only determined by the electron-transfer rate from haem a to the binuclear center , but also by the electron equilibrium between CuA and haem a. In addition , in contrast to the bovine enzyme , where the electron - and proton-transfer rates during oxidation of the fully reduced enzyme by O2 are all faster than the overall turnover rate , in the R. sphaeroides enzyme , the slowest kinetic phase was rate limiting for the overall turnover .
	manualset3
121434	19	404114	13	NULL	NULL	0	NULL	oxidation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the comparison of electron-transfer reactions in the two enzymes , we conclude that the transfer rate of the fourth electron to the binuclear center is not only determined by the electron-transfer rate from haem a to the binuclear center , but also by the electron equilibrium between CuA and haem a. In addition , in contrast to the bovine enzyme , where the electron - and proton-transfer rates during oxidation of the fully reduced enzyme by O2 are all faster than the overall turnover rate , in the R. sphaeroides enzyme , the slowest kinetic phase was rate limiting for the overall turnover .
	manualset3
121435	20	404114	13	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the comparison of electron-transfer reactions in the two enzymes , we conclude that the transfer rate of the fourth electron to the binuclear center is not only determined by the electron-transfer rate from haem a to the binuclear center , but also by the electron equilibrium between CuA and haem a. In addition , in contrast to the bovine enzyme , where the electron - and proton-transfer rates during oxidation of the fully reduced enzyme by O2 are all faster than the overall turnover rate , in the R. sphaeroides enzyme , the slowest kinetic phase was rate limiting for the overall turnover .
	manualset3
121436	21	404114	13	NULL	NULL	0	NULL	O2 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the comparison of electron-transfer reactions in the two enzymes , we conclude that the transfer rate of the fourth electron to the binuclear center is not only determined by the electron-transfer rate from haem a to the binuclear center , but also by the electron equilibrium between CuA and haem a. In addition , in contrast to the bovine enzyme , where the electron - and proton-transfer rates during oxidation of the fully reduced enzyme by O2 are all faster than the overall turnover rate , in the R. sphaeroides enzyme , the slowest kinetic phase was rate limiting for the overall turnover .
	manualset3
121437	22	404114	13	NULL	NULL	0	NULL	turnover rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the comparison of electron-transfer reactions in the two enzymes , we conclude that the transfer rate of the fourth electron to the binuclear center is not only determined by the electron-transfer rate from haem a to the binuclear center , but also by the electron equilibrium between CuA and haem a. In addition , in contrast to the bovine enzyme , where the electron - and proton-transfer rates during oxidation of the fully reduced enzyme by O2 are all faster than the overall turnover rate , in the R. sphaeroides enzyme , the slowest kinetic phase was rate limiting for the overall turnover .
	manualset3
121438	23	404114	13	NULL	NULL	0	NULL	R. sphaeroides enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the comparison of electron-transfer reactions in the two enzymes , we conclude that the transfer rate of the fourth electron to the binuclear center is not only determined by the electron-transfer rate from haem a to the binuclear center , but also by the electron equilibrium between CuA and haem a. In addition , in contrast to the bovine enzyme , where the electron - and proton-transfer rates during oxidation of the fully reduced enzyme by O2 are all faster than the overall turnover rate , in the R. sphaeroides enzyme , the slowest kinetic phase was rate limiting for the overall turnover .
	manualset3
121439	24	404114	13	NULL	NULL	0	NULL	kinetic phase 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the comparison of electron-transfer reactions in the two enzymes , we conclude that the transfer rate of the fourth electron to the binuclear center is not only determined by the electron-transfer rate from haem a to the binuclear center , but also by the electron equilibrium between CuA and haem a. In addition , in contrast to the bovine enzyme , where the electron - and proton-transfer rates during oxidation of the fully reduced enzyme by O2 are all faster than the overall turnover rate , in the R. sphaeroides enzyme , the slowest kinetic phase was rate limiting for the overall turnover .
	manualset3
121440	25	404114	13	NULL	NULL	0	NULL	rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the comparison of electron-transfer reactions in the two enzymes , we conclude that the transfer rate of the fourth electron to the binuclear center is not only determined by the electron-transfer rate from haem a to the binuclear center , but also by the electron equilibrium between CuA and haem a. In addition , in contrast to the bovine enzyme , where the electron - and proton-transfer rates during oxidation of the fully reduced enzyme by O2 are all faster than the overall turnover rate , in the R. sphaeroides enzyme , the slowest kinetic phase was rate limiting for the overall turnover .
	manualset3
121441	26	404114	13	NULL	NULL	0	NULL	turnover 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the comparison of electron-transfer reactions in the two enzymes , we conclude that the transfer rate of the fourth electron to the binuclear center is not only determined by the electron-transfer rate from haem a to the binuclear center , but also by the electron equilibrium between CuA and haem a. In addition , in contrast to the bovine enzyme , where the electron - and proton-transfer rates during oxidation of the fully reduced enzyme by O2 are all faster than the overall turnover rate , in the R. sphaeroides enzyme , the slowest kinetic phase was rate limiting for the overall turnover .
	manualset3
121442	1	404115	13	NULL	NULL	0	NULL	basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the literature and the authors ' clinical experience , the authors provide provisional recommendations for identifying and treating CYP2D6 PMs , CYP2C19 PMs , and CYP2D6 UMs .
	manualset3
121443	2	404115	13	NULL	NULL	0	NULL	literature 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the literature and the authors ' clinical experience , the authors provide provisional recommendations for identifying and treating CYP2D6 PMs , CYP2C19 PMs , and CYP2D6 UMs .
	manualset3
121444	3	404115	13	NULL	NULL	0	NULL	authors ' clinical experience	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the literature and the authors ' clinical experience , the authors provide provisional recommendations for identifying and treating CYP2D6 PMs , CYP2C19 PMs , and CYP2D6 UMs .
	manualset3
121445	4	404115	13	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the literature and the authors ' clinical experience , the authors provide provisional recommendations for identifying and treating CYP2D6 PMs , CYP2C19 PMs , and CYP2D6 UMs .
	manualset3
121446	5	404115	13	NULL	NULL	0	NULL	provisional recommendations	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the literature and the authors ' clinical experience , the authors provide provisional recommendations for identifying and treating CYP2D6 PMs , CYP2C19 PMs , and CYP2D6 UMs .
	manualset3
121447	6	404115	13	NULL	NULL	0	NULL	CYP2D6 PMs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the literature and the authors ' clinical experience , the authors provide provisional recommendations for identifying and treating CYP2D6 PMs , CYP2C19 PMs , and CYP2D6 UMs .
	manualset3
121448	7	404115	13	NULL	NULL	0	NULL	CYP2C19 PMs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the literature and the authors ' clinical experience , the authors provide provisional recommendations for identifying and treating CYP2D6 PMs , CYP2C19 PMs , and CYP2D6 UMs .
	manualset3
121449	8	404115	13	NULL	NULL	0	NULL	CYP2D6 UMs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the literature and the authors ' clinical experience , the authors provide provisional recommendations for identifying and treating CYP2D6 PMs , CYP2C19 PMs , and CYP2D6 UMs .
	manualset3
121450	1	404116	13	NULL	NULL	0	NULL	basis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the results obtained , the contribution of LMWA and soluble proteins to the PRTC and TEAC of raw , cooked , and germinated lentil seeds was calculated by multiple mean values for the content of investigated compounds and their relative potential with respect to Trolox .
	manualset3
121451	2	404116	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the results obtained , the contribution of LMWA and soluble proteins to the PRTC and TEAC of raw , cooked , and germinated lentil seeds was calculated by multiple mean values for the content of investigated compounds and their relative potential with respect to Trolox .
	manualset3
121452	3	404116	13	NULL	NULL	0	NULL	contribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the results obtained , the contribution of LMWA and soluble proteins to the PRTC and TEAC of raw , cooked , and germinated lentil seeds was calculated by multiple mean values for the content of investigated compounds and their relative potential with respect to Trolox .
	manualset3
121453	4	404116	13	NULL	NULL	0	NULL	LMWA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the results obtained , the contribution of LMWA and soluble proteins to the PRTC and TEAC of raw , cooked , and germinated lentil seeds was calculated by multiple mean values for the content of investigated compounds and their relative potential with respect to Trolox .
	manualset3
121454	5	404116	13	NULL	NULL	0	NULL	soluble proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the results obtained , the contribution of LMWA and soluble proteins to the PRTC and TEAC of raw , cooked , and germinated lentil seeds was calculated by multiple mean values for the content of investigated compounds and their relative potential with respect to Trolox .
	manualset3
121455	6	404116	13	NULL	NULL	0	NULL	PRTC 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the results obtained , the contribution of LMWA and soluble proteins to the PRTC and TEAC of raw , cooked , and germinated lentil seeds was calculated by multiple mean values for the content of investigated compounds and their relative potential with respect to Trolox .
	manualset3
121456	7	404116	13	NULL	NULL	0	NULL	TEAC	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the results obtained , the contribution of LMWA and soluble proteins to the PRTC and TEAC of raw , cooked , and germinated lentil seeds was calculated by multiple mean values for the content of investigated compounds and their relative potential with respect to Trolox .
	manualset3
121457	8	404116	13	NULL	NULL	0	NULL	lentil seeds	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the results obtained , the contribution of LMWA and soluble proteins to the PRTC and TEAC of raw , cooked , and germinated lentil seeds was calculated by multiple mean values for the content of investigated compounds and their relative potential with respect to Trolox .
	manualset3
121458	9	404116	13	NULL	NULL	0	NULL	multiple mean values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the results obtained , the contribution of LMWA and soluble proteins to the PRTC and TEAC of raw , cooked , and germinated lentil seeds was calculated by multiple mean values for the content of investigated compounds and their relative potential with respect to Trolox .
	manualset3
121459	10	404116	13	NULL	NULL	0	NULL	compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the results obtained , the contribution of LMWA and soluble proteins to the PRTC and TEAC of raw , cooked , and germinated lentil seeds was calculated by multiple mean values for the content of investigated compounds and their relative potential with respect to Trolox .
	manualset3
121460	11	404116	13	NULL	NULL	0	NULL	potential	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the results obtained , the contribution of LMWA and soluble proteins to the PRTC and TEAC of raw , cooked , and germinated lentil seeds was calculated by multiple mean values for the content of investigated compounds and their relative potential with respect to Trolox .
	manualset3
121461	12	404116	13	NULL	NULL	0	NULL	respect 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the results obtained , the contribution of LMWA and soluble proteins to the PRTC and TEAC of raw , cooked , and germinated lentil seeds was calculated by multiple mean values for the content of investigated compounds and their relative potential with respect to Trolox .
	manualset3
121462	13	404116	13	NULL	NULL	0	NULL	Trolox	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the results obtained , the contribution of LMWA and soluble proteins to the PRTC and TEAC of raw , cooked , and germinated lentil seeds was calculated by multiple mean values for the content of investigated compounds and their relative potential with respect to Trolox .
	manualset3
121463	1	404117	13	NULL	NULL	0	NULL	basis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the results of the present study , proper surveillance for colorectal cancer should be recommended for patients with endometrial carcinoma if they belong to a family with features indicative of HNPCC .
	manualset3
121464	2	404117	13	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the results of the present study , proper surveillance for colorectal cancer should be recommended for patients with endometrial carcinoma if they belong to a family with features indicative of HNPCC .
	manualset3
121465	3	404117	13	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the results of the present study , proper surveillance for colorectal cancer should be recommended for patients with endometrial carcinoma if they belong to a family with features indicative of HNPCC .
	manualset3
121466	4	404117	13	NULL	NULL	0	NULL	surveillance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the results of the present study , proper surveillance for colorectal cancer should be recommended for patients with endometrial carcinoma if they belong to a family with features indicative of HNPCC .
	manualset3
121467	5	404117	13	NULL	NULL	0	NULL	colorectal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the results of the present study , proper surveillance for colorectal cancer should be recommended for patients with endometrial carcinoma if they belong to a family with features indicative of HNPCC .
	manualset3
121468	6	404117	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the results of the present study , proper surveillance for colorectal cancer should be recommended for patients with endometrial carcinoma if they belong to a family with features indicative of HNPCC .
	manualset3
121469	7	404117	13	NULL	NULL	0	NULL	endometrial carcinoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the results of the present study , proper surveillance for colorectal cancer should be recommended for patients with endometrial carcinoma if they belong to a family with features indicative of HNPCC .
	manualset3
121470	8	404117	13	NULL	NULL	0	NULL	family	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the results of the present study , proper surveillance for colorectal cancer should be recommended for patients with endometrial carcinoma if they belong to a family with features indicative of HNPCC .
	manualset3
121471	9	404117	13	NULL	NULL	0	NULL	features 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the results of the present study , proper surveillance for colorectal cancer should be recommended for patients with endometrial carcinoma if they belong to a family with features indicative of HNPCC .
	manualset3
121472	10	404117	13	NULL	NULL	0	NULL	HNPCC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of the results of the present study , proper surveillance for colorectal cancer should be recommended for patients with endometrial carcinoma if they belong to a family with features indicative of HNPCC .
	manualset3
121473	1	404118	13	NULL	NULL	0	NULL	Blood sedimentation rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( Blood sedimentation rate and reaction times in the study of latent toxemia in pulmonary tuberculosis ) .
	manualset3
121474	2	404118	13	NULL	NULL	0	NULL	reaction times	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( Blood sedimentation rate and reaction times in the study of latent toxemia in pulmonary tuberculosis ) .
	manualset3
121475	3	404118	13	NULL	NULL	0	NULL	study	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Blood sedimentation rate and reaction times in the study of latent toxemia in pulmonary tuberculosis ) .
	manualset3
121476	4	404118	13	NULL	NULL	0	NULL	latent toxemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Blood sedimentation rate and reaction times in the study of latent toxemia in pulmonary tuberculosis ) .
	manualset3
121477	5	404118	13	NULL	NULL	0	NULL	pulmonary tuberculosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Blood sedimentation rate and reaction times in the study of latent toxemia in pulmonary tuberculosis ) .
	manualset3
121478	1	404119	13	NULL	NULL	0	NULL	delay	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A delay in the diagnosis of VUR more than 12 months after urinary tract infection ( UTI ) was also a predictive factor in an alternative model ( RR = 2.2 , 95 % CI , 1.1-6 .6 , P = 0.03 ) .
	manualset3
121479	2	404119	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A delay in the diagnosis of VUR more than 12 months after urinary tract infection ( UTI ) was also a predictive factor in an alternative model ( RR = 2.2 , 95 % CI , 1.1-6 .6 , P = 0.03 ) .
	manualset3
121480	3	404119	13	NULL	NULL	0	NULL	VUR	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A delay in the diagnosis of VUR more than 12 months after urinary tract infection ( UTI ) was also a predictive factor in an alternative model ( RR = 2.2 , 95 % CI , 1.1-6 .6 , P = 0.03 ) .
	manualset3
121481	4	404119	13	NULL	NULL	0	NULL	12 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A delay in the diagnosis of VUR more than 12 months after urinary tract infection ( UTI ) was also a predictive factor in an alternative model ( RR = 2.2 , 95 % CI , 1.1-6 .6 , P = 0.03 ) .
	manualset3
121482	5	404119	13	NULL	NULL	0	NULL	urinary tract infection ( UTI )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A delay in the diagnosis of VUR more than 12 months after urinary tract infection ( UTI ) was also a predictive factor in an alternative model ( RR = 2.2 , 95 % CI , 1.1-6 .6 , P = 0.03 ) .
	manualset3
121483	6	404119	13	NULL	NULL	0	NULL	predictive factor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A delay in the diagnosis of VUR more than 12 months after urinary tract infection ( UTI ) was also a predictive factor in an alternative model ( RR = 2.2 , 95 % CI , 1.1-6 .6 , P = 0.03 ) .
	manualset3
121484	7	404119	13	NULL	NULL	0	NULL	alternative model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A delay in the diagnosis of VUR more than 12 months after urinary tract infection ( UTI ) was also a predictive factor in an alternative model ( RR = 2.2 , 95 % CI , 1.1-6 .6 , P = 0.03 ) .
	manualset3
121485	8	404119	13	NULL	NULL	0	NULL	RR = 2.2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A delay in the diagnosis of VUR more than 12 months after urinary tract infection ( UTI ) was also a predictive factor in an alternative model ( RR = 2.2 , 95 % CI , 1.1-6 .6 , P = 0.03 ) .
	manualset3
121486	9	404119	13	NULL	NULL	0	NULL	95 % CI 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A delay in the diagnosis of VUR more than 12 months after urinary tract infection ( UTI ) was also a predictive factor in an alternative model ( RR = 2.2 , 95 % CI , 1.1-6 .6 , P = 0.03 ) .
	manualset3
121487	10	404119	13	NULL	NULL	0	NULL	1.1-6 .6 , P = 0.03	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A delay in the diagnosis of VUR more than 12 months after urinary tract infection ( UTI ) was also a predictive factor in an alternative model ( RR = 2.2 , 95 % CI , 1.1-6 .6 , P = 0.03 ) .
	manualset3
121488	1	404120	13	NULL	NULL	0	NULL	basis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these data , we anticipate that the antimetastatic agent cicaprost can be used in combination with cytostatic regimens without interfering with their clinical effectiveness .
	manualset3
121489	2	404120	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these data , we anticipate that the antimetastatic agent cicaprost can be used in combination with cytostatic regimens without interfering with their clinical effectiveness .
	manualset3
121490	3	404120	13	NULL	NULL	0	NULL	antimetastatic agent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these data , we anticipate that the antimetastatic agent cicaprost can be used in combination with cytostatic regimens without interfering with their clinical effectiveness .
	manualset3
121491	4	404120	13	NULL	NULL	0	NULL	cicaprost 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these data , we anticipate that the antimetastatic agent cicaprost can be used in combination with cytostatic regimens without interfering with their clinical effectiveness .
	manualset3
121492	5	404120	13	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these data , we anticipate that the antimetastatic agent cicaprost can be used in combination with cytostatic regimens without interfering with their clinical effectiveness .
	manualset3
121493	6	404120	13	NULL	NULL	0	NULL	cytostatic regimens	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these data , we anticipate that the antimetastatic agent cicaprost can be used in combination with cytostatic regimens without interfering with their clinical effectiveness .
	manualset3
121494	7	404120	13	NULL	NULL	0	NULL	clinical effectiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these data , we anticipate that the antimetastatic agent cicaprost can be used in combination with cytostatic regimens without interfering with their clinical effectiveness .
	manualset3
121686	1	404121	13	NULL	NULL	0	NULL	basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these excretion rates and the average frequency of occurrence of these modified ribonucleosides per cytoplasmic transfer ribonucleic acid ( residues : 2.6 dihydrouridine , 0.22 N6-threoninocarbonyladenosine , 3 pseudouridine ) as well as per cytoplasmic ribosomal ribonucleic acid ( residues : 95 pseudouridine ) , the degradation rates of transfer and ribosomal ribonucleic acids were calculated .
	manualset3
121687	2	404121	13	NULL	NULL	0	NULL	excretion rates	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these excretion rates and the average frequency of occurrence of these modified ribonucleosides per cytoplasmic transfer ribonucleic acid ( residues : 2.6 dihydrouridine , 0.22 N6-threoninocarbonyladenosine , 3 pseudouridine ) as well as per cytoplasmic ribosomal ribonucleic acid ( residues : 95 pseudouridine ) , the degradation rates of transfer and ribosomal ribonucleic acids were calculated .
	manualset3
121688	3	404121	13	NULL	NULL	0	NULL	frequency	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these excretion rates and the average frequency of occurrence of these modified ribonucleosides per cytoplasmic transfer ribonucleic acid ( residues : 2.6 dihydrouridine , 0.22 N6-threoninocarbonyladenosine , 3 pseudouridine ) as well as per cytoplasmic ribosomal ribonucleic acid ( residues : 95 pseudouridine ) , the degradation rates of transfer and ribosomal ribonucleic acids were calculated .
	manualset3
121689	4	404121	13	NULL	NULL	0	NULL	occurrence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these excretion rates and the average frequency of occurrence of these modified ribonucleosides per cytoplasmic transfer ribonucleic acid ( residues : 2.6 dihydrouridine , 0.22 N6-threoninocarbonyladenosine , 3 pseudouridine ) as well as per cytoplasmic ribosomal ribonucleic acid ( residues : 95 pseudouridine ) , the degradation rates of transfer and ribosomal ribonucleic acids were calculated .
	manualset3
121690	5	404121	13	NULL	NULL	0	NULL	ribonucleosides	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these excretion rates and the average frequency of occurrence of these modified ribonucleosides per cytoplasmic transfer ribonucleic acid ( residues : 2.6 dihydrouridine , 0.22 N6-threoninocarbonyladenosine , 3 pseudouridine ) as well as per cytoplasmic ribosomal ribonucleic acid ( residues : 95 pseudouridine ) , the degradation rates of transfer and ribosomal ribonucleic acids were calculated .
	manualset3
121691	6	404121	13	NULL	NULL	NULL	NULL	cytoplasmic transfer ribonucleic acid 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On the basis of these excretion rates and the average frequency of occurrence of these modified ribonucleosides per cytoplasmic transfer ribonucleic acid ( residues : 2.6 dihydrouridine , 0.22 N6-threoninocarbonyladenosine , 3 pseudouridine ) as well as per cytoplasmic ribosomal ribonucleic acid ( residues : 95 pseudouridine ) , the degradation rates of transfer and ribosomal ribonucleic acids were calculated .
	manualset3
121693	8	404121	13	NULL	NULL	0	NULL	residues 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these excretion rates and the average frequency of occurrence of these modified ribonucleosides per cytoplasmic transfer ribonucleic acid ( residues : 2.6 dihydrouridine , 0.22 N6-threoninocarbonyladenosine , 3 pseudouridine ) as well as per cytoplasmic ribosomal ribonucleic acid ( residues : 95 pseudouridine ) , the degradation rates of transfer and ribosomal ribonucleic acids were calculated .
	manualset3
121694	9	404121	13	NULL	NULL	0	NULL	2.6 dihydrouridine 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these excretion rates and the average frequency of occurrence of these modified ribonucleosides per cytoplasmic transfer ribonucleic acid ( residues : 2.6 dihydrouridine , 0.22 N6-threoninocarbonyladenosine , 3 pseudouridine ) as well as per cytoplasmic ribosomal ribonucleic acid ( residues : 95 pseudouridine ) , the degradation rates of transfer and ribosomal ribonucleic acids were calculated .
	manualset3
121695	10	404121	13	NULL	NULL	0	NULL	0.22 N6-threoninocarbonyladenosine	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these excretion rates and the average frequency of occurrence of these modified ribonucleosides per cytoplasmic transfer ribonucleic acid ( residues : 2.6 dihydrouridine , 0.22 N6-threoninocarbonyladenosine , 3 pseudouridine ) as well as per cytoplasmic ribosomal ribonucleic acid ( residues : 95 pseudouridine ) , the degradation rates of transfer and ribosomal ribonucleic acids were calculated .
	manualset3
121696	11	404121	13	NULL	NULL	0	NULL	3 pseudouridine 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these excretion rates and the average frequency of occurrence of these modified ribonucleosides per cytoplasmic transfer ribonucleic acid ( residues : 2.6 dihydrouridine , 0.22 N6-threoninocarbonyladenosine , 3 pseudouridine ) as well as per cytoplasmic ribosomal ribonucleic acid ( residues : 95 pseudouridine ) , the degradation rates of transfer and ribosomal ribonucleic acids were calculated .
	manualset3
121697	12	404121	13	NULL	NULL	0	NULL	cytoplasmic ribosomal ribonucleic acid	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these excretion rates and the average frequency of occurrence of these modified ribonucleosides per cytoplasmic transfer ribonucleic acid ( residues : 2.6 dihydrouridine , 0.22 N6-threoninocarbonyladenosine , 3 pseudouridine ) as well as per cytoplasmic ribosomal ribonucleic acid ( residues : 95 pseudouridine ) , the degradation rates of transfer and ribosomal ribonucleic acids were calculated .
	manualset3
121698	13	404121	13	NULL	NULL	0	NULL	residues	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these excretion rates and the average frequency of occurrence of these modified ribonucleosides per cytoplasmic transfer ribonucleic acid ( residues : 2.6 dihydrouridine , 0.22 N6-threoninocarbonyladenosine , 3 pseudouridine ) as well as per cytoplasmic ribosomal ribonucleic acid ( residues : 95 pseudouridine ) , the degradation rates of transfer and ribosomal ribonucleic acids were calculated .
	manualset3
121699	14	404121	13	NULL	NULL	0	NULL	95 pseudouridine	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these excretion rates and the average frequency of occurrence of these modified ribonucleosides per cytoplasmic transfer ribonucleic acid ( residues : 2.6 dihydrouridine , 0.22 N6-threoninocarbonyladenosine , 3 pseudouridine ) as well as per cytoplasmic ribosomal ribonucleic acid ( residues : 95 pseudouridine ) , the degradation rates of transfer and ribosomal ribonucleic acids were calculated .
	manualset3
121700	15	404121	13	NULL	NULL	0	NULL	degradation rates	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these excretion rates and the average frequency of occurrence of these modified ribonucleosides per cytoplasmic transfer ribonucleic acid ( residues : 2.6 dihydrouridine , 0.22 N6-threoninocarbonyladenosine , 3 pseudouridine ) as well as per cytoplasmic ribosomal ribonucleic acid ( residues : 95 pseudouridine ) , the degradation rates of transfer and ribosomal ribonucleic acids were calculated .
	manualset3
121701	16	404121	13	NULL	NULL	0	NULL	transfer ribonucleic acids 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these excretion rates and the average frequency of occurrence of these modified ribonucleosides per cytoplasmic transfer ribonucleic acid ( residues : 2.6 dihydrouridine , 0.22 N6-threoninocarbonyladenosine , 3 pseudouridine ) as well as per cytoplasmic ribosomal ribonucleic acid ( residues : 95 pseudouridine ) , the degradation rates of transfer and ribosomal ribonucleic acids were calculated .
	manualset3
121702	17	404121	13	NULL	NULL	0	NULL	ribosomal ribonucleic acids 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these excretion rates and the average frequency of occurrence of these modified ribonucleosides per cytoplasmic transfer ribonucleic acid ( residues : 2.6 dihydrouridine , 0.22 N6-threoninocarbonyladenosine , 3 pseudouridine ) as well as per cytoplasmic ribosomal ribonucleic acid ( residues : 95 pseudouridine ) , the degradation rates of transfer and ribosomal ribonucleic acids were calculated .
	manualset3
121703	1	404122	13	NULL	NULL	0	NULL	basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these findings , the heparan sulfate chain can be defined as a copolymer containing heparin regions in its structure .
	manualset3
121704	2	404122	13	NULL	NULL	0	NULL	findings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these findings , the heparan sulfate chain can be defined as a copolymer containing heparin regions in its structure .
	manualset3
121705	3	404122	13	NULL	NULL	0	NULL	heparan sulfate chain 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these findings , the heparan sulfate chain can be defined as a copolymer containing heparin regions in its structure .
	manualset3
121706	4	404122	13	NULL	NULL	0	NULL	copolymer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these findings , the heparan sulfate chain can be defined as a copolymer containing heparin regions in its structure .
	manualset3
121707	5	404122	13	NULL	NULL	0	NULL	heparin regions 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these findings , the heparan sulfate chain can be defined as a copolymer containing heparin regions in its structure .
	manualset3
121708	6	404122	13	NULL	NULL	0	NULL	structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these findings , the heparan sulfate chain can be defined as a copolymer containing heparin regions in its structure .
	manualset3
121709	1	404123	13	NULL	NULL	0	NULL	basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these results , a distinct + / - ROA couplet at 1335/1317 cm ( -1 ) observed in the extended amide III region is assigned to a turn in the valinomycin backbone .
	manualset3
121710	2	404123	13	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these results , a distinct + / - ROA couplet at 1335/1317 cm ( -1 ) observed in the extended amide III region is assigned to a turn in the valinomycin backbone .
	manualset3
121711	3	404123	13	NULL	NULL	0	NULL	+ / - ROA couplet 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these results , a distinct + / - ROA couplet at 1335/1317 cm ( -1 ) observed in the extended amide III region is assigned to a turn in the valinomycin backbone .
	manualset3
121712	4	404123	13	NULL	NULL	0	NULL	1335/1317 cm ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these results , a distinct + / - ROA couplet at 1335/1317 cm ( -1 ) observed in the extended amide III region is assigned to a turn in the valinomycin backbone .
	manualset3
121713	5	404123	13	NULL	NULL	0	NULL	amide III region 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these results , a distinct + / - ROA couplet at 1335/1317 cm ( -1 ) observed in the extended amide III region is assigned to a turn in the valinomycin backbone .
	manualset3
121714	6	404123	13	NULL	NULL	0	NULL	turn	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these results , a distinct + / - ROA couplet at 1335/1317 cm ( -1 ) observed in the extended amide III region is assigned to a turn in the valinomycin backbone .
	manualset3
121715	7	404123	13	NULL	NULL	0	NULL	valinomycin backbone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of these results , a distinct + / - ROA couplet at 1335/1317 cm ( -1 ) observed in the extended amide III region is assigned to a turn in the valinomycin backbone .
	manualset3
121716	1	404124	13	NULL	NULL	0	NULL	basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this correspondence for quite different types of PSII preparations exhibiting marked difference in the pH dependence of the apparent proton release pattern , it is concluded that the inhibition of the S2 -- ) S3 , S3 -- ) S0 , and S0 -- ) S1 transitions in the acidic region is an inherent property of the OEC .
	manualset3
121717	2	404124	13	NULL	NULL	0	NULL	correspondence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this correspondence for quite different types of PSII preparations exhibiting marked difference in the pH dependence of the apparent proton release pattern , it is concluded that the inhibition of the S2 -- ) S3 , S3 -- ) S0 , and S0 -- ) S1 transitions in the acidic region is an inherent property of the OEC .
	manualset3
121718	3	404124	13	NULL	NULL	0	NULL	types of PSII preparations	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this correspondence for quite different types of PSII preparations exhibiting marked difference in the pH dependence of the apparent proton release pattern , it is concluded that the inhibition of the S2 -- ) S3 , S3 -- ) S0 , and S0 -- ) S1 transitions in the acidic region is an inherent property of the OEC .
	manualset3
121719	4	404124	13	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this correspondence for quite different types of PSII preparations exhibiting marked difference in the pH dependence of the apparent proton release pattern , it is concluded that the inhibition of the S2 -- ) S3 , S3 -- ) S0 , and S0 -- ) S1 transitions in the acidic region is an inherent property of the OEC .
	manualset3
121720	5	404124	13	NULL	NULL	0	NULL	pH	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this correspondence for quite different types of PSII preparations exhibiting marked difference in the pH dependence of the apparent proton release pattern , it is concluded that the inhibition of the S2 -- ) S3 , S3 -- ) S0 , and S0 -- ) S1 transitions in the acidic region is an inherent property of the OEC .
	manualset3
121721	6	404124	13	NULL	NULL	0	NULL	dependence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this correspondence for quite different types of PSII preparations exhibiting marked difference in the pH dependence of the apparent proton release pattern , it is concluded that the inhibition of the S2 -- ) S3 , S3 -- ) S0 , and S0 -- ) S1 transitions in the acidic region is an inherent property of the OEC .
	manualset3
121723	7	404124	13	NULL	NULL	0	NULL	proton release pattern	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this correspondence for quite different types of PSII preparations exhibiting marked difference in the pH dependence of the apparent proton release pattern , it is concluded that the inhibition of the S2 -- ) S3 , S3 -- ) S0 , and S0 -- ) S1 transitions in the acidic region is an inherent property of the OEC .
	manualset3
121724	8	404124	13	NULL	NULL	0	NULL	inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this correspondence for quite different types of PSII preparations exhibiting marked difference in the pH dependence of the apparent proton release pattern , it is concluded that the inhibition of the S2 -- ) S3 , S3 -- ) S0 , and S0 -- ) S1 transitions in the acidic region is an inherent property of the OEC .
	manualset3
121725	9	404124	13	NULL	NULL	0	NULL	S2 -- ) S3 transition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this correspondence for quite different types of PSII preparations exhibiting marked difference in the pH dependence of the apparent proton release pattern , it is concluded that the inhibition of the S2 -- ) S3 , S3 -- ) S0 , and S0 -- ) S1 transitions in the acidic region is an inherent property of the OEC .
	manualset3
121726	10	404124	13	NULL	NULL	0	NULL	S3 -- ) S0 transition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this correspondence for quite different types of PSII preparations exhibiting marked difference in the pH dependence of the apparent proton release pattern , it is concluded that the inhibition of the S2 -- ) S3 , S3 -- ) S0 , and S0 -- ) S1 transitions in the acidic region is an inherent property of the OEC .
	manualset3
121727	11	404124	13	NULL	NULL	0	NULL	S0 -- ) S1 transition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this correspondence for quite different types of PSII preparations exhibiting marked difference in the pH dependence of the apparent proton release pattern , it is concluded that the inhibition of the S2 -- ) S3 , S3 -- ) S0 , and S0 -- ) S1 transitions in the acidic region is an inherent property of the OEC .
	manualset3
121728	12	404124	13	NULL	NULL	0	NULL	acidic region	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this correspondence for quite different types of PSII preparations exhibiting marked difference in the pH dependence of the apparent proton release pattern , it is concluded that the inhibition of the S2 -- ) S3 , S3 -- ) S0 , and S0 -- ) S1 transitions in the acidic region is an inherent property of the OEC .
	manualset3
121729	13	404124	13	NULL	NULL	0	NULL	property 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this correspondence for quite different types of PSII preparations exhibiting marked difference in the pH dependence of the apparent proton release pattern , it is concluded that the inhibition of the S2 -- ) S3 , S3 -- ) S0 , and S0 -- ) S1 transitions in the acidic region is an inherent property of the OEC .
	manualset3
121730	14	404124	13	NULL	NULL	0	NULL	OEC	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this correspondence for quite different types of PSII preparations exhibiting marked difference in the pH dependence of the apparent proton release pattern , it is concluded that the inhibition of the S2 -- ) S3 , S3 -- ) S0 , and S0 -- ) S1 transitions in the acidic region is an inherent property of the OEC .
	manualset3
121731	1	404125	13	NULL	NULL	0	NULL	basis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this model we suggest that in the geriatric and hyperthyroid patients there is a reduction in the number of ` membrane-units ' , that in hypokalemia and during digoxin treatment there is inhibition of the sodium-pump component of the ` membrane-units ' and that in chronic renal failure there is a decrease in the permeability of the membrane to sodium .
	manualset3
121732	2	404125	13	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this model we suggest that in the geriatric and hyperthyroid patients there is a reduction in the number of ` membrane-units ' , that in hypokalemia and during digoxin treatment there is inhibition of the sodium-pump component of the ` membrane-units ' and that in chronic renal failure there is a decrease in the permeability of the membrane to sodium .
	manualset3
121733	3	404125	13	NULL	NULL	0	NULL	geriatric patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this model we suggest that in the geriatric and hyperthyroid patients there is a reduction in the number of ` membrane-units ' , that in hypokalemia and during digoxin treatment there is inhibition of the sodium-pump component of the ` membrane-units ' and that in chronic renal failure there is a decrease in the permeability of the membrane to sodium .
	manualset3
121734	4	404125	13	NULL	NULL	0	NULL	hyperthyroid patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this model we suggest that in the geriatric and hyperthyroid patients there is a reduction in the number of ` membrane-units ' , that in hypokalemia and during digoxin treatment there is inhibition of the sodium-pump component of the ` membrane-units ' and that in chronic renal failure there is a decrease in the permeability of the membrane to sodium .
	manualset3
121735	5	404125	13	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this model we suggest that in the geriatric and hyperthyroid patients there is a reduction in the number of ` membrane-units ' , that in hypokalemia and during digoxin treatment there is inhibition of the sodium-pump component of the ` membrane-units ' and that in chronic renal failure there is a decrease in the permeability of the membrane to sodium .
	manualset3
121736	6	404125	13	NULL	NULL	0	NULL	number of ` membrane-units '	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this model we suggest that in the geriatric and hyperthyroid patients there is a reduction in the number of ` membrane-units ' , that in hypokalemia and during digoxin treatment there is inhibition of the sodium-pump component of the ` membrane-units ' and that in chronic renal failure there is a decrease in the permeability of the membrane to sodium .
	manualset3
121737	7	404125	13	NULL	NULL	0	NULL	hypokalemia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this model we suggest that in the geriatric and hyperthyroid patients there is a reduction in the number of ` membrane-units ' , that in hypokalemia and during digoxin treatment there is inhibition of the sodium-pump component of the ` membrane-units ' and that in chronic renal failure there is a decrease in the permeability of the membrane to sodium .
	manualset3
121738	8	404125	13	NULL	NULL	0	NULL	digoxin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this model we suggest that in the geriatric and hyperthyroid patients there is a reduction in the number of ` membrane-units ' , that in hypokalemia and during digoxin treatment there is inhibition of the sodium-pump component of the ` membrane-units ' and that in chronic renal failure there is a decrease in the permeability of the membrane to sodium .
	manualset3
121739	9	404125	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this model we suggest that in the geriatric and hyperthyroid patients there is a reduction in the number of ` membrane-units ' , that in hypokalemia and during digoxin treatment there is inhibition of the sodium-pump component of the ` membrane-units ' and that in chronic renal failure there is a decrease in the permeability of the membrane to sodium .
	manualset3
121740	10	404125	13	NULL	NULL	0	NULL	inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this model we suggest that in the geriatric and hyperthyroid patients there is a reduction in the number of ` membrane-units ' , that in hypokalemia and during digoxin treatment there is inhibition of the sodium-pump component of the ` membrane-units ' and that in chronic renal failure there is a decrease in the permeability of the membrane to sodium .
	manualset3
121741	11	404125	13	NULL	NULL	0	NULL	sodium-pump component	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this model we suggest that in the geriatric and hyperthyroid patients there is a reduction in the number of ` membrane-units ' , that in hypokalemia and during digoxin treatment there is inhibition of the sodium-pump component of the ` membrane-units ' and that in chronic renal failure there is a decrease in the permeability of the membrane to sodium .
	manualset3
121742	12	404125	13	NULL	NULL	0	NULL	` membrane-units ' 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this model we suggest that in the geriatric and hyperthyroid patients there is a reduction in the number of ` membrane-units ' , that in hypokalemia and during digoxin treatment there is inhibition of the sodium-pump component of the ` membrane-units ' and that in chronic renal failure there is a decrease in the permeability of the membrane to sodium .
	manualset3
121743	13	404125	13	NULL	NULL	0	NULL	chronic renal failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this model we suggest that in the geriatric and hyperthyroid patients there is a reduction in the number of ` membrane-units ' , that in hypokalemia and during digoxin treatment there is inhibition of the sodium-pump component of the ` membrane-units ' and that in chronic renal failure there is a decrease in the permeability of the membrane to sodium .
	manualset3
121744	14	404125	13	NULL	NULL	0	NULL	decrease 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this model we suggest that in the geriatric and hyperthyroid patients there is a reduction in the number of ` membrane-units ' , that in hypokalemia and during digoxin treatment there is inhibition of the sodium-pump component of the ` membrane-units ' and that in chronic renal failure there is a decrease in the permeability of the membrane to sodium .
	manualset3
121745	15	404125	13	NULL	NULL	0	NULL	permeability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this model we suggest that in the geriatric and hyperthyroid patients there is a reduction in the number of ` membrane-units ' , that in hypokalemia and during digoxin treatment there is inhibition of the sodium-pump component of the ` membrane-units ' and that in chronic renal failure there is a decrease in the permeability of the membrane to sodium .
	manualset3
121746	16	404125	13	NULL	NULL	0	NULL	membrane 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this model we suggest that in the geriatric and hyperthyroid patients there is a reduction in the number of ` membrane-units ' , that in hypokalemia and during digoxin treatment there is inhibition of the sodium-pump component of the ` membrane-units ' and that in chronic renal failure there is a decrease in the permeability of the membrane to sodium .
	manualset3
121747	17	404125	13	NULL	NULL	0	NULL	sodium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of this model we suggest that in the geriatric and hyperthyroid patients there is a reduction in the number of ` membrane-units ' , that in hypokalemia and during digoxin treatment there is inhibition of the sodium-pump component of the ` membrane-units ' and that in chronic renal failure there is a decrease in the permeability of the membrane to sodium .
	manualset3
121748	1	404126	13	NULL	NULL	0	NULL	benefit of probiotics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the benefit of probiotics in the management of pouchitis in patients underwent ileal pouch anal anastomosis : a meta-analysis of controlled clinical trials .
	manualset3
121749	2	404126	13	NULL	NULL	0	NULL	management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the benefit of probiotics in the management of pouchitis in patients underwent ileal pouch anal anastomosis : a meta-analysis of controlled clinical trials .
	manualset3
121750	3	404126	13	NULL	NULL	0	NULL	pouchitis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the benefit of probiotics in the management of pouchitis in patients underwent ileal pouch anal anastomosis : a meta-analysis of controlled clinical trials .
	manualset3
121751	4	404126	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On the benefit of probiotics in the management of pouchitis in patients underwent ileal pouch anal anastomosis : a meta-analysis of controlled clinical trials .
	manualset3
121752	5	404126	13	NULL	NULL	0	NULL	ileal pouch anal anastomosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	On the benefit of probiotics in the management of pouchitis in patients underwent ileal pouch anal anastomosis : a meta-analysis of controlled clinical trials .
	manualset3
121753	6	404126	13	NULL	NULL	0	NULL	 meta-analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the benefit of probiotics in the management of pouchitis in patients underwent ileal pouch anal anastomosis : a meta-analysis of controlled clinical trials .
	manualset3
121754	7	404126	13	NULL	NULL	0	NULL	clinical trials 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the benefit of probiotics in the management of pouchitis in patients underwent ileal pouch anal anastomosis : a meta-analysis of controlled clinical trials .
	manualset3
121776	1	404127	13	NULL	NULL	0	NULL	cohesion subscale	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the cohesion subscale , significant differences were noted between AN and BED , p & lt ; .019 , with AN scoring higher than BED .
	manualset3
121777	2	404127	13	NULL	NULL	0	NULL	differences 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	On the cohesion subscale , significant differences were noted between AN and BED , p & lt ; .019 , with AN scoring higher than BED .
	manualset3
121778	3	404127	13	NULL	NULL	0	NULL	AN	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the cohesion subscale , significant differences were noted between AN and BED , p & lt ; .019 , with AN scoring higher than BED .
	manualset3
121779	4	404127	13	NULL	NULL	0	NULL	BED	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the cohesion subscale , significant differences were noted between AN and BED , p & lt ; .019 , with AN scoring higher than BED .
	manualset3
121780	5	404127	13	NULL	NULL	0	NULL	p & lt ; .019	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the cohesion subscale , significant differences were noted between AN and BED , p & lt ; .019 , with AN scoring higher than BED .
	manualset3
121782	6	404127	13	NULL	NULL	NULL	NULL	AN 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On the cohesion subscale , significant differences were noted between AN and BED , p & lt ; .019 , with AN scoring higher than BED .
	manualset3
121784	7	404127	13	NULL	NULL	0	NULL	BED 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the cohesion subscale , significant differences were noted between AN and BED , p & lt ; .019 , with AN scoring higher than BED .
	manualset3
121789	1	404128	13	NULL	NULL	0	NULL	contralateral side	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contralateral side , young adult animals show synapse turnover similar to the ipsilateral inner molecular layer .
	manualset3
121790	2	404128	13	NULL	NULL	0	NULL	young adult animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contralateral side , young adult animals show synapse turnover similar to the ipsilateral inner molecular layer .
	manualset3
121791	3	404128	13	NULL	NULL	0	NULL	synapse turnover 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contralateral side , young adult animals show synapse turnover similar to the ipsilateral inner molecular layer .
	manualset3
121792	4	404128	13	NULL	NULL	0	NULL	 ipsilateral inner molecular layer	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contralateral side , young adult animals show synapse turnover similar to the ipsilateral inner molecular layer .
	manualset3
121793	1	404129	13	NULL	NULL	0	NULL	contrary	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , ( 3 ) J ( C6/8-H 1 ' ) follows the usual trans to cis ratio ( ( 3 ) J ( C-H ( cis ) ) & lt ; ( 3 ) J ( C-H ( trans ) ) ) for purine nucleosides , but reveals the opposite relation ( ( 3 ) J ( C-H ( cis ) ) ) ( 3 ) J ( C-H ( trans ) ) ) for pyrimidine nucleosides .
	manualset3
121794	2	404129	13	NULL	NULL	0	NULL	( 3 ) J ( C6/8-H 1 ' )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , ( 3 ) J ( C6/8-H 1 ' ) follows the usual trans to cis ratio ( ( 3 ) J ( C-H ( cis ) ) & lt ; ( 3 ) J ( C-H ( trans ) ) ) for purine nucleosides , but reveals the opposite relation ( ( 3 ) J ( C-H ( cis ) ) ) ( 3 ) J ( C-H ( trans ) ) ) for pyrimidine nucleosides .
	manualset3
121795	3	404129	13	NULL	NULL	0	NULL	trans to cis ratio	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , ( 3 ) J ( C6/8-H 1 ' ) follows the usual trans to cis ratio ( ( 3 ) J ( C-H ( cis ) ) & lt ; ( 3 ) J ( C-H ( trans ) ) ) for purine nucleosides , but reveals the opposite relation ( ( 3 ) J ( C-H ( cis ) ) ) ( 3 ) J ( C-H ( trans ) ) ) for pyrimidine nucleosides .
	manualset3
121796	4	404129	13	NULL	NULL	0	NULL	( ( 3 ) J ( C-H ( cis ) ) & lt ; ( 3 ) J ( C-H ( trans ) ) )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , ( 3 ) J ( C6/8-H 1 ' ) follows the usual trans to cis ratio ( ( 3 ) J ( C-H ( cis ) ) & lt ; ( 3 ) J ( C-H ( trans ) ) ) for purine nucleosides , but reveals the opposite relation ( ( 3 ) J ( C-H ( cis ) ) ) ( 3 ) J ( C-H ( trans ) ) ) for pyrimidine nucleosides .
	manualset3
121797	5	404129	13	NULL	NULL	0	NULL	purine nucleosides	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , ( 3 ) J ( C6/8-H 1 ' ) follows the usual trans to cis ratio ( ( 3 ) J ( C-H ( cis ) ) & lt ; ( 3 ) J ( C-H ( trans ) ) ) for purine nucleosides , but reveals the opposite relation ( ( 3 ) J ( C-H ( cis ) ) ) ( 3 ) J ( C-H ( trans ) ) ) for pyrimidine nucleosides .
	manualset3
121798	6	404129	13	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , ( 3 ) J ( C6/8-H 1 ' ) follows the usual trans to cis ratio ( ( 3 ) J ( C-H ( cis ) ) & lt ; ( 3 ) J ( C-H ( trans ) ) ) for purine nucleosides , but reveals the opposite relation ( ( 3 ) J ( C-H ( cis ) ) ) ( 3 ) J ( C-H ( trans ) ) ) for pyrimidine nucleosides .
	manualset3
121799	7	404129	13	NULL	NULL	0	NULL	( ( 3 ) J ( C-H ( cis ) ) ) ( 3 ) J ( C-H ( trans ) ) ) 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , ( 3 ) J ( C6/8-H 1 ' ) follows the usual trans to cis ratio ( ( 3 ) J ( C-H ( cis ) ) & lt ; ( 3 ) J ( C-H ( trans ) ) ) for purine nucleosides , but reveals the opposite relation ( ( 3 ) J ( C-H ( cis ) ) ) ( 3 ) J ( C-H ( trans ) ) ) for pyrimidine nucleosides .
	manualset3
121800	8	404129	13	NULL	NULL	0	NULL	pyrimidine nucleosides	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , ( 3 ) J ( C6/8-H 1 ' ) follows the usual trans to cis ratio ( ( 3 ) J ( C-H ( cis ) ) & lt ; ( 3 ) J ( C-H ( trans ) ) ) for purine nucleosides , but reveals the opposite relation ( ( 3 ) J ( C-H ( cis ) ) ) ( 3 ) J ( C-H ( trans ) ) ) for pyrimidine nucleosides .
	manualset3
121801	1	404130	13	NULL	NULL	0	NULL	delta-sleep-inducing peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	A delta-sleep-inducing peptide in various concentrations inhibits the pharmacological activity of trypsin and pronase E under experimental conditions .
	manualset3
121802	2	404130	13	NULL	NULL	0	NULL	concentrations 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A delta-sleep-inducing peptide in various concentrations inhibits the pharmacological activity of trypsin and pronase E under experimental conditions .
	manualset3
121803	3	404130	13	NULL	NULL	0	NULL	pharmacological activity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A delta-sleep-inducing peptide in various concentrations inhibits the pharmacological activity of trypsin and pronase E under experimental conditions .
	manualset3
121804	4	404130	13	NULL	NULL	0	NULL	trypsin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A delta-sleep-inducing peptide in various concentrations inhibits the pharmacological activity of trypsin and pronase E under experimental conditions .
	manualset3
121805	5	404130	13	NULL	NULL	0	NULL	pronase E 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A delta-sleep-inducing peptide in various concentrations inhibits the pharmacological activity of trypsin and pronase E under experimental conditions .
	manualset3
121806	6	404130	13	NULL	NULL	0	NULL	experimental conditions 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A delta-sleep-inducing peptide in various concentrations inhibits the pharmacological activity of trypsin and pronase E under experimental conditions .
	manualset3
121813	1	404131	13	NULL	NULL	0	NULL	contrary	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , extracts from primary layers of LTMCs contained 3 times more AcSDKP ; however , after treatment of primary layers by collagenase , AcSDKP level fell to 1 pMol per 10 ( 6 ) cells .
	manualset3
121814	2	404131	13	NULL	NULL	0	NULL	extracts from primary layers of LTMCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , extracts from primary layers of LTMCs contained 3 times more AcSDKP ; however , after treatment of primary layers by collagenase , AcSDKP level fell to 1 pMol per 10 ( 6 ) cells .
	manualset3
121815	3	404131	13	NULL	NULL	0	NULL	3 times	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , extracts from primary layers of LTMCs contained 3 times more AcSDKP ; however , after treatment of primary layers by collagenase , AcSDKP level fell to 1 pMol per 10 ( 6 ) cells .
	manualset3
121816	4	404131	13	NULL	NULL	0	NULL	AcSDKP	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , extracts from primary layers of LTMCs contained 3 times more AcSDKP ; however , after treatment of primary layers by collagenase , AcSDKP level fell to 1 pMol per 10 ( 6 ) cells .
	manualset3
121817	5	404131	13	NULL	NULL	0	NULL	treatment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , extracts from primary layers of LTMCs contained 3 times more AcSDKP ; however , after treatment of primary layers by collagenase , AcSDKP level fell to 1 pMol per 10 ( 6 ) cells .
	manualset3
121818	6	404131	13	NULL	NULL	0	NULL	primary layers	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , extracts from primary layers of LTMCs contained 3 times more AcSDKP ; however , after treatment of primary layers by collagenase , AcSDKP level fell to 1 pMol per 10 ( 6 ) cells .
	manualset3
121819	7	404131	13	NULL	NULL	0	NULL	collagenase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , extracts from primary layers of LTMCs contained 3 times more AcSDKP ; however , after treatment of primary layers by collagenase , AcSDKP level fell to 1 pMol per 10 ( 6 ) cells .
	manualset3
121820	8	404131	13	NULL	NULL	0	NULL	AcSDKP level 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , extracts from primary layers of LTMCs contained 3 times more AcSDKP ; however , after treatment of primary layers by collagenase , AcSDKP level fell to 1 pMol per 10 ( 6 ) cells .
	manualset3
121821	9	404131	13	NULL	NULL	0	NULL	1 pMol per 10 ( 6 ) cells	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , extracts from primary layers of LTMCs contained 3 times more AcSDKP ; however , after treatment of primary layers by collagenase , AcSDKP level fell to 1 pMol per 10 ( 6 ) cells .
	manualset3
121822	1	404132	13	NULL	NULL	0	NULL	contrary	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , helper T-cell function was resistant to 2000 rad .
	manualset3
121823	2	404132	13	NULL	NULL	0	NULL	helper T-cell function 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , helper T-cell function was resistant to 2000 rad .
	manualset3
121824	3	404132	13	NULL	NULL	0	NULL	2000 rad	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , helper T-cell function was resistant to 2000 rad .
	manualset3
121825	1	404133	13	NULL	NULL	0	NULL	contrary	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , replacement of N2 with sulfur hexafluoride ( SF6 ) augmented the effect of hypoxia .
	manualset3
121826	2	404133	13	NULL	NULL	0	NULL	replacement of N2	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , replacement of N2 with sulfur hexafluoride ( SF6 ) augmented the effect of hypoxia .
	manualset3
121827	3	404133	13	NULL	NULL	0	NULL	sulfur hexafluoride ( SF6 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , replacement of N2 with sulfur hexafluoride ( SF6 ) augmented the effect of hypoxia .
	manualset3
121828	4	404133	13	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , replacement of N2 with sulfur hexafluoride ( SF6 ) augmented the effect of hypoxia .
	manualset3
121829	5	404133	13	NULL	NULL	0	NULL	hypoxia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , replacement of N2 with sulfur hexafluoride ( SF6 ) augmented the effect of hypoxia .
	manualset3
121830	1	404134	13	NULL	NULL	0	NULL	contrary	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , that of peritoneal dissemination was more increased in gastric cancer than in colorectal cancer ( p & lt ; 0.01 ) .
	manualset3
121831	2	404134	13	NULL	NULL	0	NULL	peritoneal dissemination 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , that of peritoneal dissemination was more increased in gastric cancer than in colorectal cancer ( p & lt ; 0.01 ) .
	manualset3
121832	3	404134	13	NULL	NULL	0	NULL	gastric cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , that of peritoneal dissemination was more increased in gastric cancer than in colorectal cancer ( p & lt ; 0.01 ) .
	manualset3
121833	4	404134	13	NULL	NULL	0	NULL	colorectal cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , that of peritoneal dissemination was more increased in gastric cancer than in colorectal cancer ( p & lt ; 0.01 ) .
	manualset3
121834	5	404134	13	NULL	NULL	0	NULL	p & lt ; 0.01 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , that of peritoneal dissemination was more increased in gastric cancer than in colorectal cancer ( p & lt ; 0.01 ) .
	manualset3
121835	1	404135	13	NULL	NULL	0	NULL	contrary	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , thymocytes had higher percentages of CD4 - CD8 + lymphocytes at 2 and 4 DPI and reached comparable levels at 8 DPI in controls and SRV-infected poults .
	manualset3
121836	2	404135	13	NULL	NULL	0	NULL	thymocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , thymocytes had higher percentages of CD4 - CD8 + lymphocytes at 2 and 4 DPI and reached comparable levels at 8 DPI in controls and SRV-infected poults .
	manualset3
121837	3	404135	13	NULL	NULL	0	NULL	percentages 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , thymocytes had higher percentages of CD4 - CD8 + lymphocytes at 2 and 4 DPI and reached comparable levels at 8 DPI in controls and SRV-infected poults .
	manualset3
121838	4	404135	13	NULL	NULL	0	NULL	CD4 -lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , thymocytes had higher percentages of CD4 - CD8 + lymphocytes at 2 and 4 DPI and reached comparable levels at 8 DPI in controls and SRV-infected poults .
	manualset3
121839	5	404135	13	NULL	NULL	0	NULL	CD8 + lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , thymocytes had higher percentages of CD4 - CD8 + lymphocytes at 2 and 4 DPI and reached comparable levels at 8 DPI in controls and SRV-infected poults .
	manualset3
121840	6	404135	13	NULL	NULL	0	NULL	2 DPI 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , thymocytes had higher percentages of CD4 - CD8 + lymphocytes at 2 and 4 DPI and reached comparable levels at 8 DPI in controls and SRV-infected poults .
	manualset3
121841	7	404135	13	NULL	NULL	0	NULL	4 DPI	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , thymocytes had higher percentages of CD4 - CD8 + lymphocytes at 2 and 4 DPI and reached comparable levels at 8 DPI in controls and SRV-infected poults .
	manualset3
121842	8	404135	13	NULL	NULL	0	NULL	levels 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , thymocytes had higher percentages of CD4 - CD8 + lymphocytes at 2 and 4 DPI and reached comparable levels at 8 DPI in controls and SRV-infected poults .
	manualset3
121843	9	404135	13	NULL	NULL	0	NULL	8 DPI 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , thymocytes had higher percentages of CD4 - CD8 + lymphocytes at 2 and 4 DPI and reached comparable levels at 8 DPI in controls and SRV-infected poults .
	manualset3
121844	10	404135	13	NULL	NULL	0	NULL	controls	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , thymocytes had higher percentages of CD4 - CD8 + lymphocytes at 2 and 4 DPI and reached comparable levels at 8 DPI in controls and SRV-infected poults .
	manualset3
121845	11	404135	13	NULL	NULL	0	NULL	SRV-infected poults 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , thymocytes had higher percentages of CD4 - CD8 + lymphocytes at 2 and 4 DPI and reached comparable levels at 8 DPI in controls and SRV-infected poults .
	manualset3
121846	1	404136	13	NULL	NULL	0	NULL	efferent nerve impulses 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the efferent nerve impulses in frog 's dorso-cutaneous nerves caused by cutaneous stimulation .
	manualset3
121847	2	404136	13	NULL	NULL	0	NULL	frog 's	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On the efferent nerve impulses in frog 's dorso-cutaneous nerves caused by cutaneous stimulation .
	manualset3
121848	3	404136	13	NULL	NULL	0	NULL	dorso-cutaneous nerves	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	On the efferent nerve impulses in frog 's dorso-cutaneous nerves caused by cutaneous stimulation .
	manualset3
121849	4	404136	13	NULL	NULL	0	NULL	cutaneous stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the efferent nerve impulses in frog 's dorso-cutaneous nerves caused by cutaneous stimulation .
	manualset3
121850	1	404137	13	NULL	NULL	0	NULL	denouement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A denouement will require a full understanding of ( 1 ) the origin and pathogenetic contribution of antibody to intrinsic factor ; ( 2 ) the connection , if any , between H. pylori infection and Type A autoimmune gastritis ; and ( 3 ) the genetic contributions to gastritis , whether due to autoimmunity or to H. pylori infection .
	manualset3
121851	2	404137	13	NULL	NULL	0	NULL	understanding 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A denouement will require a full understanding of ( 1 ) the origin and pathogenetic contribution of antibody to intrinsic factor ; ( 2 ) the connection , if any , between H. pylori infection and Type A autoimmune gastritis ; and ( 3 ) the genetic contributions to gastritis , whether due to autoimmunity or to H. pylori infection .
	manualset3
121852	3	404137	13	NULL	NULL	0	NULL	origin	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A denouement will require a full understanding of ( 1 ) the origin and pathogenetic contribution of antibody to intrinsic factor ; ( 2 ) the connection , if any , between H. pylori infection and Type A autoimmune gastritis ; and ( 3 ) the genetic contributions to gastritis , whether due to autoimmunity or to H. pylori infection .
	manualset3
121853	4	404137	13	NULL	NULL	0	NULL	pathogenetic contribution	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A denouement will require a full understanding of ( 1 ) the origin and pathogenetic contribution of antibody to intrinsic factor ; ( 2 ) the connection , if any , between H. pylori infection and Type A autoimmune gastritis ; and ( 3 ) the genetic contributions to gastritis , whether due to autoimmunity or to H. pylori infection .
	manualset3
121854	5	404137	13	NULL	NULL	0	NULL	antibody 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A denouement will require a full understanding of ( 1 ) the origin and pathogenetic contribution of antibody to intrinsic factor ; ( 2 ) the connection , if any , between H. pylori infection and Type A autoimmune gastritis ; and ( 3 ) the genetic contributions to gastritis , whether due to autoimmunity or to H. pylori infection .
	manualset3
121855	6	404137	13	NULL	NULL	0	NULL	intrinsic factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A denouement will require a full understanding of ( 1 ) the origin and pathogenetic contribution of antibody to intrinsic factor ; ( 2 ) the connection , if any , between H. pylori infection and Type A autoimmune gastritis ; and ( 3 ) the genetic contributions to gastritis , whether due to autoimmunity or to H. pylori infection .
	manualset3
121856	7	404137	13	NULL	NULL	0	NULL	connection	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A denouement will require a full understanding of ( 1 ) the origin and pathogenetic contribution of antibody to intrinsic factor ; ( 2 ) the connection , if any , between H. pylori infection and Type A autoimmune gastritis ; and ( 3 ) the genetic contributions to gastritis , whether due to autoimmunity or to H. pylori infection .
	manualset3
121857	8	404137	13	NULL	NULL	0	NULL	H. pylori infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A denouement will require a full understanding of ( 1 ) the origin and pathogenetic contribution of antibody to intrinsic factor ; ( 2 ) the connection , if any , between H. pylori infection and Type A autoimmune gastritis ; and ( 3 ) the genetic contributions to gastritis , whether due to autoimmunity or to H. pylori infection .
	manualset3
121858	9	404137	13	NULL	NULL	0	NULL	Type A autoimmune gastritis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A denouement will require a full understanding of ( 1 ) the origin and pathogenetic contribution of antibody to intrinsic factor ; ( 2 ) the connection , if any , between H. pylori infection and Type A autoimmune gastritis ; and ( 3 ) the genetic contributions to gastritis , whether due to autoimmunity or to H. pylori infection .
	manualset3
121859	10	404137	13	NULL	NULL	0	NULL	genetic contributions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A denouement will require a full understanding of ( 1 ) the origin and pathogenetic contribution of antibody to intrinsic factor ; ( 2 ) the connection , if any , between H. pylori infection and Type A autoimmune gastritis ; and ( 3 ) the genetic contributions to gastritis , whether due to autoimmunity or to H. pylori infection .
	manualset3
121860	11	404137	13	NULL	NULL	0	NULL	gastritis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A denouement will require a full understanding of ( 1 ) the origin and pathogenetic contribution of antibody to intrinsic factor ; ( 2 ) the connection , if any , between H. pylori infection and Type A autoimmune gastritis ; and ( 3 ) the genetic contributions to gastritis , whether due to autoimmunity or to H. pylori infection .
	manualset3
121861	12	404137	13	NULL	NULL	0	NULL	autoimmunity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A denouement will require a full understanding of ( 1 ) the origin and pathogenetic contribution of antibody to intrinsic factor ; ( 2 ) the connection , if any , between H. pylori infection and Type A autoimmune gastritis ; and ( 3 ) the genetic contributions to gastritis , whether due to autoimmunity or to H. pylori infection .
	manualset3
121862	13	404137	13	NULL	NULL	0	NULL	H. pylori infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A denouement will require a full understanding of ( 1 ) the origin and pathogenetic contribution of antibody to intrinsic factor ; ( 2 ) the connection , if any , between H. pylori infection and Type A autoimmune gastritis ; and ( 3 ) the genetic contributions to gastritis , whether due to autoimmunity or to H. pylori infection .
	manualset3
121863	1	404138	13	NULL	NULL	0	NULL	guinea-pig 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On the guinea-pig isolated ileum ( 10 ( -5 ) M ) and trachea ( 10 ( -6 ) M ) , indoramin is devoid of anticholinergic activity , but has a potent antihistamine action which satisfies the criteria for competitive antagonism ; the pA ( 2 ) value for this antagonism on the ileum is 8.2.5 .
	manualset3
121864	2	404138	13	NULL	NULL	0	NULL	ileum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	On the guinea-pig isolated ileum ( 10 ( -5 ) M ) and trachea ( 10 ( -6 ) M ) , indoramin is devoid of anticholinergic activity , but has a potent antihistamine action which satisfies the criteria for competitive antagonism ; the pA ( 2 ) value for this antagonism on the ileum is 8.2.5 .
	manualset3
121865	3	404138	13	NULL	NULL	0	NULL	10 ( -5 ) M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the guinea-pig isolated ileum ( 10 ( -5 ) M ) and trachea ( 10 ( -6 ) M ) , indoramin is devoid of anticholinergic activity , but has a potent antihistamine action which satisfies the criteria for competitive antagonism ; the pA ( 2 ) value for this antagonism on the ileum is 8.2.5 .
	manualset3
121866	4	404138	13	NULL	NULL	0	NULL	trachea	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	On the guinea-pig isolated ileum ( 10 ( -5 ) M ) and trachea ( 10 ( -6 ) M ) , indoramin is devoid of anticholinergic activity , but has a potent antihistamine action which satisfies the criteria for competitive antagonism ; the pA ( 2 ) value for this antagonism on the ileum is 8.2.5 .
	manualset3
121867	5	404138	13	NULL	NULL	0	NULL	10 ( -6 ) M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the guinea-pig isolated ileum ( 10 ( -5 ) M ) and trachea ( 10 ( -6 ) M ) , indoramin is devoid of anticholinergic activity , but has a potent antihistamine action which satisfies the criteria for competitive antagonism ; the pA ( 2 ) value for this antagonism on the ileum is 8.2.5 .
	manualset3
121868	6	404138	13	NULL	NULL	0	NULL	indoramin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	On the guinea-pig isolated ileum ( 10 ( -5 ) M ) and trachea ( 10 ( -6 ) M ) , indoramin is devoid of anticholinergic activity , but has a potent antihistamine action which satisfies the criteria for competitive antagonism ; the pA ( 2 ) value for this antagonism on the ileum is 8.2.5 .
	manualset3
121869	7	404138	13	NULL	NULL	0	NULL	anticholinergic activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the guinea-pig isolated ileum ( 10 ( -5 ) M ) and trachea ( 10 ( -6 ) M ) , indoramin is devoid of anticholinergic activity , but has a potent antihistamine action which satisfies the criteria for competitive antagonism ; the pA ( 2 ) value for this antagonism on the ileum is 8.2.5 .
	manualset3
121870	8	404138	13	NULL	NULL	0	NULL	antihistamine action 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the guinea-pig isolated ileum ( 10 ( -5 ) M ) and trachea ( 10 ( -6 ) M ) , indoramin is devoid of anticholinergic activity , but has a potent antihistamine action which satisfies the criteria for competitive antagonism ; the pA ( 2 ) value for this antagonism on the ileum is 8.2.5 .
	manualset3
121871	9	404138	13	NULL	NULL	0	NULL	criteria	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the guinea-pig isolated ileum ( 10 ( -5 ) M ) and trachea ( 10 ( -6 ) M ) , indoramin is devoid of anticholinergic activity , but has a potent antihistamine action which satisfies the criteria for competitive antagonism ; the pA ( 2 ) value for this antagonism on the ileum is 8.2.5 .
	manualset3
121872	10	404138	13	NULL	NULL	NULL	NULL	competitive antagonism	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On the guinea-pig isolated ileum ( 10 ( -5 ) M ) and trachea ( 10 ( -6 ) M ) , indoramin is devoid of anticholinergic activity , but has a potent antihistamine action which satisfies the criteria for competitive antagonism ; the pA ( 2 ) value for this antagonism on the ileum is 8.2.5 .
	manualset3
121873	11	404138	13	NULL	NULL	0	NULL	pA ( 2 ) value	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the guinea-pig isolated ileum ( 10 ( -5 ) M ) and trachea ( 10 ( -6 ) M ) , indoramin is devoid of anticholinergic activity , but has a potent antihistamine action which satisfies the criteria for competitive antagonism ; the pA ( 2 ) value for this antagonism on the ileum is 8.2.5 .
	manualset3
121874	12	404138	13	NULL	NULL	NULL	NULL	antagonism	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On the guinea-pig isolated ileum ( 10 ( -5 ) M ) and trachea ( 10 ( -6 ) M ) , indoramin is devoid of anticholinergic activity , but has a potent antihistamine action which satisfies the criteria for competitive antagonism ; the pA ( 2 ) value for this antagonism on the ileum is 8.2.5 .
	manualset3
121875	13	404138	13	NULL	NULL	0	NULL	ileum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	On the guinea-pig isolated ileum ( 10 ( -5 ) M ) and trachea ( 10 ( -6 ) M ) , indoramin is devoid of anticholinergic activity , but has a potent antihistamine action which satisfies the criteria for competitive antagonism ; the pA ( 2 ) value for this antagonism on the ileum is 8.2.5 .
	manualset3
121876	14	404138	13	NULL	NULL	0	NULL	8.2.5	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the guinea-pig isolated ileum ( 10 ( -5 ) M ) and trachea ( 10 ( -6 ) M ) , indoramin is devoid of anticholinergic activity , but has a potent antihistamine action which satisfies the criteria for competitive antagonism ; the pA ( 2 ) value for this antagonism on the ileum is 8.2.5 .
	manualset3
121882	1	404139	13	NULL	NULL	0	NULL	mechanism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the mechanism of cross-tolerance between morphine - and nicotine-induced antinociception : involvement of calcium channels .
	manualset3
121884	2	404139	13	NULL	NULL	0	NULL	cross-tolerance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the mechanism of cross-tolerance between morphine - and nicotine-induced antinociception : involvement of calcium channels .
	manualset3
121885	3	404139	13	NULL	NULL	0	NULL	morphine-induced antinociception	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the mechanism of cross-tolerance between morphine - and nicotine-induced antinociception : involvement of calcium channels .
	manualset3
121886	4	404139	13	NULL	NULL	0	NULL	nicotine-induced antinociception	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the mechanism of cross-tolerance between morphine - and nicotine-induced antinociception : involvement of calcium channels .
	manualset3
121887	5	404139	13	NULL	NULL	0	NULL	involvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the mechanism of cross-tolerance between morphine - and nicotine-induced antinociception : involvement of calcium channels .
	manualset3
121888	6	404139	13	NULL	NULL	0	NULL	calcium channels	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	On the mechanism of cross-tolerance between morphine - and nicotine-induced antinociception : involvement of calcium channels .
	manualset3
121889	1	404140	13	NULL	NULL	0	NULL	exposure 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the next after exposure of the cortex to DC , the dominant recovered after application of 7 -- 10 trials of geniculate stimulation .
	manualset3
121890	2	404140	13	NULL	NULL	0	NULL	cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	On the next after exposure of the cortex to DC , the dominant recovered after application of 7 -- 10 trials of geniculate stimulation .
	manualset3
121891	3	404140	13	NULL	NULL	0	NULL	DC 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	On the next after exposure of the cortex to DC , the dominant recovered after application of 7 -- 10 trials of geniculate stimulation .
	manualset3
121892	4	404140	13	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the next after exposure of the cortex to DC , the dominant recovered after application of 7 -- 10 trials of geniculate stimulation .
	manualset3
121893	5	404140	13	NULL	NULL	0	NULL	7 -- 10 trials	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the next after exposure of the cortex to DC , the dominant recovered after application of 7 -- 10 trials of geniculate stimulation .
	manualset3
121894	6	404140	13	NULL	NULL	0	NULL	geniculate stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the next after exposure of the cortex to DC , the dominant recovered after application of 7 -- 10 trials of geniculate stimulation .
	manualset3
121895	1	404141	13	NULL	NULL	0	NULL	occasion	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	On the occasion of examining Rh genotype of our patient it was established that , instead of previous Rh genotype inherited from his father , after retransplantation he had a new Rh phenotype acquired from his brother who inherited it from their mother .
	manualset3
121896	2	404141	13	NULL	NULL	0	NULL	Rh genotype	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the occasion of examining Rh genotype of our patient it was established that , instead of previous Rh genotype inherited from his father , after retransplantation he had a new Rh phenotype acquired from his brother who inherited it from their mother .
	manualset3
121897	3	404141	13	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	On the occasion of examining Rh genotype of our patient it was established that , instead of previous Rh genotype inherited from his father , after retransplantation he had a new Rh phenotype acquired from his brother who inherited it from their mother .
	manualset3
121898	4	404141	13	NULL	NULL	0	NULL	Rh genotype	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the occasion of examining Rh genotype of our patient it was established that , instead of previous Rh genotype inherited from his father , after retransplantation he had a new Rh phenotype acquired from his brother who inherited it from their mother .
	manualset3
121899	5	404141	13	NULL	NULL	0	NULL	father	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	On the occasion of examining Rh genotype of our patient it was established that , instead of previous Rh genotype inherited from his father , after retransplantation he had a new Rh phenotype acquired from his brother who inherited it from their mother .
	manualset3
121900	6	404141	13	NULL	NULL	0	NULL	retransplantation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	On the occasion of examining Rh genotype of our patient it was established that , instead of previous Rh genotype inherited from his father , after retransplantation he had a new Rh phenotype acquired from his brother who inherited it from their mother .
	manualset3
121901	7	404141	13	NULL	NULL	0	NULL	Rh phenotype	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the occasion of examining Rh genotype of our patient it was established that , instead of previous Rh genotype inherited from his father , after retransplantation he had a new Rh phenotype acquired from his brother who inherited it from their mother .
	manualset3
121902	8	404141	13	NULL	NULL	0	NULL	brother	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	On the occasion of examining Rh genotype of our patient it was established that , instead of previous Rh genotype inherited from his father , after retransplantation he had a new Rh phenotype acquired from his brother who inherited it from their mother .
	manualset3
121903	9	404141	13	NULL	NULL	0	NULL	mother	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	On the occasion of examining Rh genotype of our patient it was established that , instead of previous Rh genotype inherited from his father , after retransplantation he had a new Rh phenotype acquired from his brother who inherited it from their mother .
	manualset3
121904	1	404142	13	NULL	NULL	0	NULL	optical properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the optical properties of the imidazolium ionic liquids .
	manualset3
121905	2	404142	13	NULL	NULL	0	NULL	imidazolium ionic liquids 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the optical properties of the imidazolium ionic liquids .
	manualset3
121906	1	404143	13	NULL	NULL	0	NULL	2-5A-dependent RNase ( RNase L ) activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , 2-5A-dependent RNase ( RNase L ) activity in Lz cells was low , being about 10-20 % of that of L929 cells .
	manualset3
121907	2	404143	13	NULL	NULL	0	NULL	Lz cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , 2-5A-dependent RNase ( RNase L ) activity in Lz cells was low , being about 10-20 % of that of L929 cells .
	manualset3
121908	3	404143	13	NULL	NULL	0	NULL	10-20 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , 2-5A-dependent RNase ( RNase L ) activity in Lz cells was low , being about 10-20 % of that of L929 cells .
	manualset3
121909	4	404143	13	NULL	NULL	0	NULL	L929 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , 2-5A-dependent RNase ( RNase L ) activity in Lz cells was low , being about 10-20 % of that of L929 cells .
	manualset3
121910	1	404144	13	NULL	NULL	0	NULL	ACE inhibition 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , ACE inhibition has been shown to induce neocapillarization in hypertrophied myocardium .
	manualset3
121911	2	404144	13	NULL	NULL	0	NULL	neocapillarization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , ACE inhibition has been shown to induce neocapillarization in hypertrophied myocardium .
	manualset3
121912	3	404144	13	NULL	NULL	0	NULL	 hypertrophied myocardium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , ACE inhibition has been shown to induce neocapillarization in hypertrophied myocardium .
	manualset3
121914	1	404145	13	NULL	NULL	0	NULL	BSP transport 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , BSP transport was inhibited by approximately 50 % by 10 microM corticosterone sulfate , spironolactone , and several other steroids .
	manualset3
121915	2	404145	13	NULL	NULL	0	NULL	approximately 50 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , BSP transport was inhibited by approximately 50 % by 10 microM corticosterone sulfate , spironolactone , and several other steroids .
	manualset3
121916	3	404145	13	NULL	NULL	0	NULL	10 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , BSP transport was inhibited by approximately 50 % by 10 microM corticosterone sulfate , spironolactone , and several other steroids .
	manualset3
121920	4	404145	13	NULL	NULL	0	NULL	corticosterone sulfate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , BSP transport was inhibited by approximately 50 % by 10 microM corticosterone sulfate , spironolactone , and several other steroids .
	manualset3
121921	5	404145	13	NULL	NULL	0	NULL	spironolactone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , BSP transport was inhibited by approximately 50 % by 10 microM corticosterone sulfate , spironolactone , and several other steroids .
	manualset3
121922	6	404145	13	NULL	NULL	0	NULL	steroids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , BSP transport was inhibited by approximately 50 % by 10 microM corticosterone sulfate , spironolactone , and several other steroids .
	manualset3
121932	1	404146	13	NULL	NULL	0	NULL	HIP complexes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , HIP complexes between alendronate and TBAI showed the maximum hydrophobicity at the same molar ratio at pH 10.3 .
	manualset3
121934	2	404146	13	NULL	NULL	0	NULL	alendronate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , HIP complexes between alendronate and TBAI showed the maximum hydrophobicity at the same molar ratio at pH 10.3 .
	manualset3
121936	3	404146	13	NULL	NULL	0	NULL	TBAI	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , HIP complexes between alendronate and TBAI showed the maximum hydrophobicity at the same molar ratio at pH 10.3 .
	manualset3
121937	4	404146	13	NULL	NULL	0	NULL	hydrophobicity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , HIP complexes between alendronate and TBAI showed the maximum hydrophobicity at the same molar ratio at pH 10.3 .
	manualset3
121938	5	404146	13	NULL	NULL	0	NULL	molar ratio	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , HIP complexes between alendronate and TBAI showed the maximum hydrophobicity at the same molar ratio at pH 10.3 .
	manualset3
121939	6	404146	13	NULL	NULL	0	NULL	pH 10.3	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , HIP complexes between alendronate and TBAI showed the maximum hydrophobicity at the same molar ratio at pH 10.3 .
	manualset3
121942	1	404147	13	NULL	NULL	0	NULL	density-functional approach	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A density-functional approach and canonical Monte Carlo simulations are presented for describing the ionic microscopic structure around the DNA molecule immersed in mixed-size counterion solutions .
	manualset3
121943	2	404147	13	NULL	NULL	0	NULL	canonical Monte Carlo simulations	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A density-functional approach and canonical Monte Carlo simulations are presented for describing the ionic microscopic structure around the DNA molecule immersed in mixed-size counterion solutions .
	manualset3
121944	3	404147	13	NULL	NULL	0	NULL	 ionic microscopic structure	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A density-functional approach and canonical Monte Carlo simulations are presented for describing the ionic microscopic structure around the DNA molecule immersed in mixed-size counterion solutions .
	manualset3
121945	4	404147	13	NULL	NULL	0	NULL	DNA molecule 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A density-functional approach and canonical Monte Carlo simulations are presented for describing the ionic microscopic structure around the DNA molecule immersed in mixed-size counterion solutions .
	manualset3
121946	5	404147	13	NULL	NULL	0	NULL	counterion solutions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A density-functional approach and canonical Monte Carlo simulations are presented for describing the ionic microscopic structure around the DNA molecule immersed in mixed-size counterion solutions .
	manualset3
121949	1	404148	13	NULL	NULL	0	NULL	class	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , another class of previously reported gamma-secretase modulators , naphthyl ketones , inhibited SPP activity as well as selective proteolysis by gamma-secretase .
	manualset3
121950	2	404148	13	NULL	NULL	0	NULL	gamma-secretase modulators	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , another class of previously reported gamma-secretase modulators , naphthyl ketones , inhibited SPP activity as well as selective proteolysis by gamma-secretase .
	manualset3
121951	3	404148	13	NULL	NULL	0	NULL	naphthyl ketones	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , another class of previously reported gamma-secretase modulators , naphthyl ketones , inhibited SPP activity as well as selective proteolysis by gamma-secretase .
	manualset3
121953	4	404148	13	NULL	NULL	0	NULL	SPP activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , another class of previously reported gamma-secretase modulators , naphthyl ketones , inhibited SPP activity as well as selective proteolysis by gamma-secretase .
	manualset3
121954	5	404148	13	NULL	NULL	0	NULL	proteolysis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , another class of previously reported gamma-secretase modulators , naphthyl ketones , inhibited SPP activity as well as selective proteolysis by gamma-secretase .
	manualset3
121955	6	404148	13	NULL	NULL	0	NULL	gamma-secretase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , another class of previously reported gamma-secretase modulators , naphthyl ketones , inhibited SPP activity as well as selective proteolysis by gamma-secretase .
	manualset3
121984	1	404149	13	NULL	NULL	0	NULL	collections of A. ovale adults	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , collections of A. ovale adults on wild Felidae were higher ( 18.3 % ) than findings of A. aureolatum ( 9.2 % ) .
	manualset3
121994	2	404149	13	NULL	NULL	0	NULL	wild Felidae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , collections of A. ovale adults on wild Felidae were higher ( 18.3 % ) than findings of A. aureolatum ( 9.2 % ) .
	manualset3
121995	3	404149	13	NULL	NULL	0	NULL	18.3 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , collections of A. ovale adults on wild Felidae were higher ( 18.3 % ) than findings of A. aureolatum ( 9.2 % ) .
	manualset3
121996	4	404149	13	NULL	NULL	0	NULL	A. aureolatum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , collections of A. ovale adults on wild Felidae were higher ( 18.3 % ) than findings of A. aureolatum ( 9.2 % ) .
	manualset3
121998	5	404149	13	NULL	NULL	0	NULL	9.2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , collections of A. ovale adults on wild Felidae were higher ( 18.3 % ) than findings of A. aureolatum ( 9.2 % ) .
	manualset3
122003	1	404150	13	NULL	NULL	0	NULL	condoms	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , condoms have a failure rate of 9-12 % for 1st year use , but increased skill effectiveness is increased .
	manualset3
122004	2	404150	13	NULL	NULL	0	NULL	failure rate 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , condoms have a failure rate of 9-12 % for 1st year use , but increased skill effectiveness is increased .
	manualset3
122005	3	404150	13	NULL	NULL	0	NULL	9-12 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , condoms have a failure rate of 9-12 % for 1st year use , but increased skill effectiveness is increased .
	manualset3
122006	4	404150	13	NULL	NULL	0	NULL	1st year 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , condoms have a failure rate of 9-12 % for 1st year use , but increased skill effectiveness is increased .
	manualset3
122007	5	404150	13	NULL	NULL	0	NULL	use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , condoms have a failure rate of 9-12 % for 1st year use , but increased skill effectiveness is increased .
	manualset3
122008	6	404150	13	NULL	NULL	0	NULL	skill effectiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , condoms have a failure rate of 9-12 % for 1st year use , but increased skill effectiveness is increased .
	manualset3
122010	1	404151	13	NULL	NULL	0	NULL	dialkylalkyne	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , dialkylalkyne inserted into a zirconium-silene complex gave silazirconacyclopentene 9 .
	manualset3
122011	2	404151	13	NULL	NULL	0	NULL	zirconium-silene complex	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , dialkylalkyne inserted into a zirconium-silene complex gave silazirconacyclopentene 9 .
	manualset3
122012	3	404151	13	NULL	NULL	0	NULL	silazirconacyclopentene 9	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , dialkylalkyne inserted into a zirconium-silene complex gave silazirconacyclopentene 9 .
	manualset3
122020	1	404152	13	NULL	NULL	0	NULL	doses	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , given in the same doses as in the acid-secretory studies , PHA stimulated pancreatic amylase secretion in rats prepared with chronic pancreatic cannula .
	manualset3
122021	2	404152	13	NULL	NULL	0	NULL	acid-secretory studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , given in the same doses as in the acid-secretory studies , PHA stimulated pancreatic amylase secretion in rats prepared with chronic pancreatic cannula .
	manualset3
122027	3	404152	13	NULL	NULL	0	NULL	PHA	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , given in the same doses as in the acid-secretory studies , PHA stimulated pancreatic amylase secretion in rats prepared with chronic pancreatic cannula .
	manualset3
122029	4	404152	13	NULL	NULL	0	NULL	pancreatic amylase secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , given in the same doses as in the acid-secretory studies , PHA stimulated pancreatic amylase secretion in rats prepared with chronic pancreatic cannula .
	manualset3
122031	5	404152	13	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , given in the same doses as in the acid-secretory studies , PHA stimulated pancreatic amylase secretion in rats prepared with chronic pancreatic cannula .
	manualset3
122032	6	404152	13	NULL	NULL	0	NULL	chronic pancreatic cannula	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , given in the same doses as in the acid-secretory studies , PHA stimulated pancreatic amylase secretion in rats prepared with chronic pancreatic cannula .
	manualset3
122037	1	404153	13	NULL	NULL	0	NULL	neuropeptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , it has been reported that various neuropeptides not only influence the neuroendocrine compound of sleep , but also exert specific effects on the sleep electroencephalogram ( EEG ) .
	manualset3
122040	2	404153	13	NULL	NULL	0	NULL	influence 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , it has been reported that various neuropeptides not only influence the neuroendocrine compound of sleep , but also exert specific effects on the sleep electroencephalogram ( EEG ) .
	manualset3
122041	3	404153	13	NULL	NULL	0	NULL	neuroendocrine compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , it has been reported that various neuropeptides not only influence the neuroendocrine compound of sleep , but also exert specific effects on the sleep electroencephalogram ( EEG ) .
	manualset3
122042	4	404153	13	NULL	NULL	0	NULL	sleep	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , it has been reported that various neuropeptides not only influence the neuroendocrine compound of sleep , but also exert specific effects on the sleep electroencephalogram ( EEG ) .
	manualset3
122044	5	404153	13	NULL	NULL	0	NULL	effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , it has been reported that various neuropeptides not only influence the neuroendocrine compound of sleep , but also exert specific effects on the sleep electroencephalogram ( EEG ) .
	manualset3
125242	6	404153	13	NULL	NULL	0	NULL	sleep electroencephalogram ( EEG ) 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , it has been reported that various neuropeptides not only influence the neuroendocrine compound of sleep , but also exert specific effects on the sleep electroencephalogram ( EEG ) .
	manualset3
122045	6	404154	13	NULL	NULL	NULL	NULL	left-left composites	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On the other hand , left-left composites were not consistently judged by subjects with and without chimpanzee experience as the most similar to the whole original face , which might be explained as the result of an attentional bias in the human observers towards the right side of the chimpanzee expressions .
	manualset3
122064	7	404154	13	NULL	NULL	0	NULL	subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , left-left composites were not consistently judged by subjects with and without chimpanzee experience as the most similar to the whole original face , which might be explained as the result of an attentional bias in the human observers towards the right side of the chimpanzee expressions .
	manualset3
122065	8	404154	13	NULL	NULL	0	NULL	chimpanzee	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , left-left composites were not consistently judged by subjects with and without chimpanzee experience as the most similar to the whole original face , which might be explained as the result of an attentional bias in the human observers towards the right side of the chimpanzee expressions .
	manualset3
122070	9	404154	13	NULL	NULL	0	NULL	experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , left-left composites were not consistently judged by subjects with and without chimpanzee experience as the most similar to the whole original face , which might be explained as the result of an attentional bias in the human observers towards the right side of the chimpanzee expressions .
	manualset3
122072	10	404154	13	NULL	NULL	0	NULL	original face	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , left-left composites were not consistently judged by subjects with and without chimpanzee experience as the most similar to the whole original face , which might be explained as the result of an attentional bias in the human observers towards the right side of the chimpanzee expressions .
	manualset3
122075	11	404154	13	NULL	NULL	0	NULL	result	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , left-left composites were not consistently judged by subjects with and without chimpanzee experience as the most similar to the whole original face , which might be explained as the result of an attentional bias in the human observers towards the right side of the chimpanzee expressions .
	manualset3
122077	12	404154	13	NULL	NULL	0	NULL	attentional bias	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , left-left composites were not consistently judged by subjects with and without chimpanzee experience as the most similar to the whole original face , which might be explained as the result of an attentional bias in the human observers towards the right side of the chimpanzee expressions .
	manualset3
122084	13	404154	13	NULL	NULL	0	NULL	human observers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , left-left composites were not consistently judged by subjects with and without chimpanzee experience as the most similar to the whole original face , which might be explained as the result of an attentional bias in the human observers towards the right side of the chimpanzee expressions .
	manualset3
122085	14	404154	13	NULL	NULL	0	NULL	right side	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , left-left composites were not consistently judged by subjects with and without chimpanzee experience as the most similar to the whole original face , which might be explained as the result of an attentional bias in the human observers towards the right side of the chimpanzee expressions .
	manualset3
122086	15	404154	13	NULL	NULL	0	NULL	chimpanzee expressions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , left-left composites were not consistently judged by subjects with and without chimpanzee experience as the most similar to the whole original face , which might be explained as the result of an attentional bias in the human observers towards the right side of the chimpanzee expressions .
	manualset3
122087	1	404155	13	NULL	NULL	0	NULL	mAb 59D8 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , mAb 59D8 , specific for GHRPL at the beta-chain NH2-terminus of fibrin , reacted with the ( DD ) E complex in a dose-dependent manner .
	manualset3
122088	2	404155	13	NULL	NULL	0	NULL	GHRPL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , mAb 59D8 , specific for GHRPL at the beta-chain NH2-terminus of fibrin , reacted with the ( DD ) E complex in a dose-dependent manner .
	manualset3
122089	3	404155	13	NULL	NULL	0	NULL	beta-chain NH2-terminus of fibrin	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , mAb 59D8 , specific for GHRPL at the beta-chain NH2-terminus of fibrin , reacted with the ( DD ) E complex in a dose-dependent manner .
	manualset3
122093	4	404155	13	NULL	NULL	0	NULL	( DD ) E complex	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , mAb 59D8 , specific for GHRPL at the beta-chain NH2-terminus of fibrin , reacted with the ( DD ) E complex in a dose-dependent manner .
	manualset3
122094	5	404155	13	NULL	NULL	0	NULL	dose-dependent manner	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , mAb 59D8 , specific for GHRPL at the beta-chain NH2-terminus of fibrin , reacted with the ( DD ) E complex in a dose-dependent manner .
	manualset3
122099	1	404156	13	NULL	NULL	0	NULL	BPTI 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A derivative of BPTI containing only the 5-55 disulfide bond , termed ( 5-55 ) Ala , has been shown previously to fold into a structure very similar to that of native BPTI and to be a functional trypsin inhibitor .
	manualset3
122100	2	404156	13	NULL	NULL	0	NULL	5-55 disulfide bond	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A derivative of BPTI containing only the 5-55 disulfide bond , termed ( 5-55 ) Ala , has been shown previously to fold into a structure very similar to that of native BPTI and to be a functional trypsin inhibitor .
	manualset3
122101	3	404156	13	NULL	NULL	NULL	NULL	( 5-55 ) Ala	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A derivative of BPTI containing only the 5-55 disulfide bond , termed ( 5-55 ) Ala , has been shown previously to fold into a structure very similar to that of native BPTI and to be a functional trypsin inhibitor .
	manualset3
122102	4	404156	13	NULL	NULL	0	NULL	structure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A derivative of BPTI containing only the 5-55 disulfide bond , termed ( 5-55 ) Ala , has been shown previously to fold into a structure very similar to that of native BPTI and to be a functional trypsin inhibitor .
	manualset3
122103	5	404156	13	NULL	NULL	0	NULL	native BPTI	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A derivative of BPTI containing only the 5-55 disulfide bond , termed ( 5-55 ) Ala , has been shown previously to fold into a structure very similar to that of native BPTI and to be a functional trypsin inhibitor .
	manualset3
122104	6	404156	13	NULL	NULL	0	NULL	functional trypsin inhibitor 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A derivative of BPTI containing only the 5-55 disulfide bond , termed ( 5-55 ) Ala , has been shown previously to fold into a structure very similar to that of native BPTI and to be a functional trypsin inhibitor .
	manualset3
122105	1	404157	13	NULL	NULL	0	NULL	murine fibroblast ( L929 ) cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , murine fibroblast ( L929 ) cells are known to be deficient in cell-cell adhesive proteins and therefore lack gap junctions for cellular communication .
	manualset3
122106	2	404157	13	NULL	NULL	0	NULL	cell-cell adhesive proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , murine fibroblast ( L929 ) cells are known to be deficient in cell-cell adhesive proteins and therefore lack gap junctions for cellular communication .
	manualset3
122107	3	404157	13	NULL	NULL	0	NULL	gap junctions 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , murine fibroblast ( L929 ) cells are known to be deficient in cell-cell adhesive proteins and therefore lack gap junctions for cellular communication .
	manualset3
122108	4	404157	13	NULL	NULL	0	NULL	 cellular communication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , murine fibroblast ( L929 ) cells are known to be deficient in cell-cell adhesive proteins and therefore lack gap junctions for cellular communication .
	manualset3
122130	1	404158	13	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , no significant difference between the rats with and without chlorobenzene was observed as regards cysteine levels at 24 h. Hepatic glutamate , glycine , methionine and serine levels were unaltered but hepatic taurine levels were significantly decreased by the chlorobenzene at both 6 and 24 h. Chlorobenzene administration had no effect on hepatic cystathionine synthase and cystathionase activities .
	manualset3
122131	2	404158	13	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , no significant difference between the rats with and without chlorobenzene was observed as regards cysteine levels at 24 h. Hepatic glutamate , glycine , methionine and serine levels were unaltered but hepatic taurine levels were significantly decreased by the chlorobenzene at both 6 and 24 h. Chlorobenzene administration had no effect on hepatic cystathionine synthase and cystathionase activities .
	manualset3
122133	3	404158	13	NULL	NULL	0	NULL	chlorobenzene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , no significant difference between the rats with and without chlorobenzene was observed as regards cysteine levels at 24 h. Hepatic glutamate , glycine , methionine and serine levels were unaltered but hepatic taurine levels were significantly decreased by the chlorobenzene at both 6 and 24 h. Chlorobenzene administration had no effect on hepatic cystathionine synthase and cystathionase activities .
	manualset3
122134	4	404158	13	NULL	NULL	0	NULL	cysteine levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , no significant difference between the rats with and without chlorobenzene was observed as regards cysteine levels at 24 h. Hepatic glutamate , glycine , methionine and serine levels were unaltered but hepatic taurine levels were significantly decreased by the chlorobenzene at both 6 and 24 h. Chlorobenzene administration had no effect on hepatic cystathionine synthase and cystathionase activities .
	manualset3
122136	5	404158	13	NULL	NULL	0	NULL	24 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , no significant difference between the rats with and without chlorobenzene was observed as regards cysteine levels at 24 h. Hepatic glutamate , glycine , methionine and serine levels were unaltered but hepatic taurine levels were significantly decreased by the chlorobenzene at both 6 and 24 h. Chlorobenzene administration had no effect on hepatic cystathionine synthase and cystathionase activities .
	manualset3
122138	6	404158	13	NULL	NULL	NULL	NULL	Hepatic glutamate levels	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On the other hand , no significant difference between the rats with and without chlorobenzene was observed as regards cysteine levels at 24 h. Hepatic glutamate , glycine , methionine and serine levels were unaltered but hepatic taurine levels were significantly decreased by the chlorobenzene at both 6 and 24 h. Chlorobenzene administration had no effect on hepatic cystathionine synthase and cystathionase activities .
	manualset3
122146	7	404158	13	NULL	NULL	0	NULL	glycine levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , no significant difference between the rats with and without chlorobenzene was observed as regards cysteine levels at 24 h. Hepatic glutamate , glycine , methionine and serine levels were unaltered but hepatic taurine levels were significantly decreased by the chlorobenzene at both 6 and 24 h. Chlorobenzene administration had no effect on hepatic cystathionine synthase and cystathionase activities .
	manualset3
122147	8	404158	13	NULL	NULL	0	NULL	methionine levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , no significant difference between the rats with and without chlorobenzene was observed as regards cysteine levels at 24 h. Hepatic glutamate , glycine , methionine and serine levels were unaltered but hepatic taurine levels were significantly decreased by the chlorobenzene at both 6 and 24 h. Chlorobenzene administration had no effect on hepatic cystathionine synthase and cystathionase activities .
	manualset3
122148	9	404158	13	NULL	NULL	0	NULL	serine levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , no significant difference between the rats with and without chlorobenzene was observed as regards cysteine levels at 24 h. Hepatic glutamate , glycine , methionine and serine levels were unaltered but hepatic taurine levels were significantly decreased by the chlorobenzene at both 6 and 24 h. Chlorobenzene administration had no effect on hepatic cystathionine synthase and cystathionase activities .
	manualset3
122149	10	404158	13	NULL	NULL	0	NULL	hepatic taurine levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , no significant difference between the rats with and without chlorobenzene was observed as regards cysteine levels at 24 h. Hepatic glutamate , glycine , methionine and serine levels were unaltered but hepatic taurine levels were significantly decreased by the chlorobenzene at both 6 and 24 h. Chlorobenzene administration had no effect on hepatic cystathionine synthase and cystathionase activities .
	manualset3
122150	11	404158	13	NULL	NULL	0	NULL	chlorobenzene 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , no significant difference between the rats with and without chlorobenzene was observed as regards cysteine levels at 24 h. Hepatic glutamate , glycine , methionine and serine levels were unaltered but hepatic taurine levels were significantly decreased by the chlorobenzene at both 6 and 24 h. Chlorobenzene administration had no effect on hepatic cystathionine synthase and cystathionase activities .
	manualset3
122151	12	404158	13	NULL	NULL	0	NULL	6 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , no significant difference between the rats with and without chlorobenzene was observed as regards cysteine levels at 24 h. Hepatic glutamate , glycine , methionine and serine levels were unaltered but hepatic taurine levels were significantly decreased by the chlorobenzene at both 6 and 24 h. Chlorobenzene administration had no effect on hepatic cystathionine synthase and cystathionase activities .
	manualset3
122152	13	404158	13	NULL	NULL	0	NULL	24 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , no significant difference between the rats with and without chlorobenzene was observed as regards cysteine levels at 24 h. Hepatic glutamate , glycine , methionine and serine levels were unaltered but hepatic taurine levels were significantly decreased by the chlorobenzene at both 6 and 24 h. Chlorobenzene administration had no effect on hepatic cystathionine synthase and cystathionase activities .
	manualset3
122153	14	404158	13	NULL	NULL	0	NULL	Chlorobenzene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , no significant difference between the rats with and without chlorobenzene was observed as regards cysteine levels at 24 h. Hepatic glutamate , glycine , methionine and serine levels were unaltered but hepatic taurine levels were significantly decreased by the chlorobenzene at both 6 and 24 h. Chlorobenzene administration had no effect on hepatic cystathionine synthase and cystathionase activities .
	manualset3
122154	15	404158	13	NULL	NULL	0	NULL	administration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , no significant difference between the rats with and without chlorobenzene was observed as regards cysteine levels at 24 h. Hepatic glutamate , glycine , methionine and serine levels were unaltered but hepatic taurine levels were significantly decreased by the chlorobenzene at both 6 and 24 h. Chlorobenzene administration had no effect on hepatic cystathionine synthase and cystathionase activities .
	manualset3
122155	16	404158	13	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , no significant difference between the rats with and without chlorobenzene was observed as regards cysteine levels at 24 h. Hepatic glutamate , glycine , methionine and serine levels were unaltered but hepatic taurine levels were significantly decreased by the chlorobenzene at both 6 and 24 h. Chlorobenzene administration had no effect on hepatic cystathionine synthase and cystathionase activities .
	manualset3
122156	17	404158	13	NULL	NULL	0	NULL	hepatic cystathionine synthase activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , no significant difference between the rats with and without chlorobenzene was observed as regards cysteine levels at 24 h. Hepatic glutamate , glycine , methionine and serine levels were unaltered but hepatic taurine levels were significantly decreased by the chlorobenzene at both 6 and 24 h. Chlorobenzene administration had no effect on hepatic cystathionine synthase and cystathionase activities .
	manualset3
122157	18	404158	13	NULL	NULL	0	NULL	cystathionase activities 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , no significant difference between the rats with and without chlorobenzene was observed as regards cysteine levels at 24 h. Hepatic glutamate , glycine , methionine and serine levels were unaltered but hepatic taurine levels were significantly decreased by the chlorobenzene at both 6 and 24 h. Chlorobenzene administration had no effect on hepatic cystathionine synthase and cystathionase activities .
	manualset3
122158	1	404159	13	NULL	NULL	0	NULL	levels of Tg	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , only the levels of Tg increased significantly in peritoneal dialysate .
	manualset3
122159	2	404159	13	NULL	NULL	0	NULL	peritoneal dialysate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , only the levels of Tg increased significantly in peritoneal dialysate .
	manualset3
122160	1	404160	13	NULL	NULL	0	NULL	political leverage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , political leverage by the tobacco industry , exercised through various policy functions , intimidated the government leadership and eventually controlled its actions .
	manualset3
122161	2	404160	13	NULL	NULL	0	NULL	tobacco industry	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , political leverage by the tobacco industry , exercised through various policy functions , intimidated the government leadership and eventually controlled its actions .
	manualset3
122162	3	404160	13	NULL	NULL	0	NULL	policy functions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , political leverage by the tobacco industry , exercised through various policy functions , intimidated the government leadership and eventually controlled its actions .
	manualset3
122163	4	404160	13	NULL	NULL	0	NULL	government leadership	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , political leverage by the tobacco industry , exercised through various policy functions , intimidated the government leadership and eventually controlled its actions .
	manualset3
122164	5	404160	13	NULL	NULL	0	NULL	actions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , political leverage by the tobacco industry , exercised through various policy functions , intimidated the government leadership and eventually controlled its actions .
	manualset3
122165	1	404161	13	NULL	NULL	0	NULL	size-exclusion chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , size-exclusion chromatography of reconstituted Zn7 - or Cd7-metallothionein revealed the presence of monomeric and dimeric species .
	manualset3
122166	2	404161	13	NULL	NULL	0	NULL	Zn7 -metallothionein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , size-exclusion chromatography of reconstituted Zn7 - or Cd7-metallothionein revealed the presence of monomeric and dimeric species .
	manualset3
122167	3	404161	13	NULL	NULL	0	NULL	Cd7-metallothionein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , size-exclusion chromatography of reconstituted Zn7 - or Cd7-metallothionein revealed the presence of monomeric and dimeric species .
	manualset3
122168	4	404161	13	NULL	NULL	0	NULL	monomeric species 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , size-exclusion chromatography of reconstituted Zn7 - or Cd7-metallothionein revealed the presence of monomeric and dimeric species .
	manualset3
122169	5	404161	13	NULL	NULL	0	NULL	dimeric species	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , size-exclusion chromatography of reconstituted Zn7 - or Cd7-metallothionein revealed the presence of monomeric and dimeric species .
	manualset3
122170	1	404162	13	NULL	NULL	0	NULL	tandospirone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , tandospirone exerted no potentiating effect on the shortening of sleep latency induced by p-chlorophenylalanine .
	manualset3
122171	2	404162	13	NULL	NULL	0	NULL	effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , tandospirone exerted no potentiating effect on the shortening of sleep latency induced by p-chlorophenylalanine .
	manualset3
122172	3	404162	13	NULL	NULL	0	NULL	sleep latency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , tandospirone exerted no potentiating effect on the shortening of sleep latency induced by p-chlorophenylalanine .
	manualset3
122173	4	404162	13	NULL	NULL	0	NULL	p-chlorophenylalanine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , tandospirone exerted no potentiating effect on the shortening of sleep latency induced by p-chlorophenylalanine .
	manualset3
122174	1	404163	13	NULL	NULL	NULL	NULL	blood 	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On the other hand , the blood levels of TNF-alpha , IL-6 , IL-8 , and MIP-1 alpha were correlated with the severity and mortality in patients with sepsis .
	manualset3
122175	2	404163	13	NULL	NULL	0	NULL	levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the blood levels of TNF-alpha , IL-6 , IL-8 , and MIP-1 alpha were correlated with the severity and mortality in patients with sepsis .
	manualset3
122176	3	404163	13	NULL	NULL	0	NULL	TNF-alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the blood levels of TNF-alpha , IL-6 , IL-8 , and MIP-1 alpha were correlated with the severity and mortality in patients with sepsis .
	manualset3
122177	4	404163	13	NULL	NULL	0	NULL	IL-6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the blood levels of TNF-alpha , IL-6 , IL-8 , and MIP-1 alpha were correlated with the severity and mortality in patients with sepsis .
	manualset3
122178	5	404163	13	NULL	NULL	0	NULL	IL-8	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the blood levels of TNF-alpha , IL-6 , IL-8 , and MIP-1 alpha were correlated with the severity and mortality in patients with sepsis .
	manualset3
122179	6	404163	13	NULL	NULL	0	NULL	MIP-1 alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the blood levels of TNF-alpha , IL-6 , IL-8 , and MIP-1 alpha were correlated with the severity and mortality in patients with sepsis .
	manualset3
122180	7	404163	13	NULL	NULL	0	NULL	severity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the blood levels of TNF-alpha , IL-6 , IL-8 , and MIP-1 alpha were correlated with the severity and mortality in patients with sepsis .
	manualset3
122181	8	404163	13	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the blood levels of TNF-alpha , IL-6 , IL-8 , and MIP-1 alpha were correlated with the severity and mortality in patients with sepsis .
	manualset3
122182	9	404163	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the blood levels of TNF-alpha , IL-6 , IL-8 , and MIP-1 alpha were correlated with the severity and mortality in patients with sepsis .
	manualset3
122183	10	404163	13	NULL	NULL	0	NULL	sepsis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the blood levels of TNF-alpha , IL-6 , IL-8 , and MIP-1 alpha were correlated with the severity and mortality in patients with sepsis .
	manualset3
122184	1	404164	13	NULL	NULL	0	NULL	cell attachment activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the cell attachment activity of IGFBP-rP1 was markedly increased by the proteolytic processing .
	manualset3
122185	2	404164	13	NULL	NULL	0	NULL	IGFBP-rP1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the cell attachment activity of IGFBP-rP1 was markedly increased by the proteolytic processing .
	manualset3
122186	3	404164	13	NULL	NULL	0	NULL	proteolytic processing	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the cell attachment activity of IGFBP-rP1 was markedly increased by the proteolytic processing .
	manualset3
122187	1	404165	13	NULL	NULL	0	NULL	co-existence mechanism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the co-existence mechanism of fearfulness and boldness is also considered .
	manualset3
122188	2	404165	13	NULL	NULL	0	NULL	fearfulness 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the co-existence mechanism of fearfulness and boldness is also considered .
	manualset3
122189	3	404165	13	NULL	NULL	0	NULL	boldness	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the co-existence mechanism of fearfulness and boldness is also considered .
	manualset3
122190	1	404166	13	NULL	NULL	0	NULL	description	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A description of the GABAergic neurons and axon terminals in the motor nuclei of the cat thalamus .
	manualset3
122191	2	404166	13	NULL	NULL	0	NULL	GABAergic neurons 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A description of the GABAergic neurons and axon terminals in the motor nuclei of the cat thalamus .
	manualset3
122192	3	404166	13	NULL	NULL	0	NULL	axon terminals	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A description of the GABAergic neurons and axon terminals in the motor nuclei of the cat thalamus .
	manualset3
122193	4	404166	13	NULL	NULL	0	NULL	motor nuclei	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A description of the GABAergic neurons and axon terminals in the motor nuclei of the cat thalamus .
	manualset3
122194	5	404166	13	NULL	NULL	0	NULL	cat thalamus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A description of the GABAergic neurons and axon terminals in the motor nuclei of the cat thalamus .
	manualset3
122195	1	404167	13	NULL	NULL	0	NULL	impact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the impact of the variability of CETP gene on HDL cholesterol variations in Caucasians is controversial .
	manualset3
122196	2	404167	13	NULL	NULL	0	NULL	variability 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the impact of the variability of CETP gene on HDL cholesterol variations in Caucasians is controversial .
	manualset3
122197	3	404167	13	NULL	NULL	0	NULL	CETP gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the impact of the variability of CETP gene on HDL cholesterol variations in Caucasians is controversial .
	manualset3
122198	4	404167	13	NULL	NULL	0	NULL	HDL cholesterol variations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the impact of the variability of CETP gene on HDL cholesterol variations in Caucasians is controversial .
	manualset3
122199	5	404167	13	NULL	NULL	0	NULL	Caucasians 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the impact of the variability of CETP gene on HDL cholesterol variations in Caucasians is controversial .
	manualset3
122200	1	404168	13	NULL	NULL	0	NULL	occurrence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the occurrence of empty fungal hyphae , surrounded or trapped in amorphous material , in samples from Si + plants suggests that phenolic-like compounds or phytoalexins played a primary role in rice defense response against infection by M. grisea .
	manualset3
122201	2	404168	13	NULL	NULL	0	NULL	empty fungal hyphae	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the occurrence of empty fungal hyphae , surrounded or trapped in amorphous material , in samples from Si + plants suggests that phenolic-like compounds or phytoalexins played a primary role in rice defense response against infection by M. grisea .
	manualset3
122202	3	404168	13	NULL	NULL	0	NULL	amorphous material 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the occurrence of empty fungal hyphae , surrounded or trapped in amorphous material , in samples from Si + plants suggests that phenolic-like compounds or phytoalexins played a primary role in rice defense response against infection by M. grisea .
	manualset3
122203	4	404168	13	NULL	NULL	0	NULL	samples	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the occurrence of empty fungal hyphae , surrounded or trapped in amorphous material , in samples from Si + plants suggests that phenolic-like compounds or phytoalexins played a primary role in rice defense response against infection by M. grisea .
	manualset3
122204	5	404168	13	NULL	NULL	0	NULL	Si + plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the occurrence of empty fungal hyphae , surrounded or trapped in amorphous material , in samples from Si + plants suggests that phenolic-like compounds or phytoalexins played a primary role in rice defense response against infection by M. grisea .
	manualset3
122205	6	404168	13	NULL	NULL	0	NULL	phenolic-like compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the occurrence of empty fungal hyphae , surrounded or trapped in amorphous material , in samples from Si + plants suggests that phenolic-like compounds or phytoalexins played a primary role in rice defense response against infection by M. grisea .
	manualset3
122206	7	404168	13	NULL	NULL	0	NULL	phytoalexins 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the occurrence of empty fungal hyphae , surrounded or trapped in amorphous material , in samples from Si + plants suggests that phenolic-like compounds or phytoalexins played a primary role in rice defense response against infection by M. grisea .
	manualset3
122207	8	404168	13	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the occurrence of empty fungal hyphae , surrounded or trapped in amorphous material , in samples from Si + plants suggests that phenolic-like compounds or phytoalexins played a primary role in rice defense response against infection by M. grisea .
	manualset3
122208	9	404168	13	NULL	NULL	NULL	NULL	rice defense response	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On the other hand , the occurrence of empty fungal hyphae , surrounded or trapped in amorphous material , in samples from Si + plants suggests that phenolic-like compounds or phytoalexins played a primary role in rice defense response against infection by M. grisea .
	manualset3
122209	10	404168	13	NULL	NULL	0	NULL	infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the occurrence of empty fungal hyphae , surrounded or trapped in amorphous material , in samples from Si + plants suggests that phenolic-like compounds or phytoalexins played a primary role in rice defense response against infection by M. grisea .
	manualset3
122210	11	404168	13	NULL	NULL	0	NULL	M. grisea 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the occurrence of empty fungal hyphae , surrounded or trapped in amorphous material , in samples from Si + plants suggests that phenolic-like compounds or phytoalexins played a primary role in rice defense response against infection by M. grisea .
	manualset3
122211	1	404169	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the presence of a shared environmental effect in addition to a major gene component does not alter the detection of the major gene nor the transmission probability estimates , which are close to the expected Mendelian values .
	manualset3
122212	2	404169	13	NULL	NULL	0	NULL	environmental effect 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the presence of a shared environmental effect in addition to a major gene component does not alter the detection of the major gene nor the transmission probability estimates , which are close to the expected Mendelian values .
	manualset3
122213	3	404169	13	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the presence of a shared environmental effect in addition to a major gene component does not alter the detection of the major gene nor the transmission probability estimates , which are close to the expected Mendelian values .
	manualset3
122214	4	404169	13	NULL	NULL	NULL	NULL	major gene component 	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On the other hand , the presence of a shared environmental effect in addition to a major gene component does not alter the detection of the major gene nor the transmission probability estimates , which are close to the expected Mendelian values .
	manualset3
122215	5	404169	13	NULL	NULL	0	NULL	detection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the presence of a shared environmental effect in addition to a major gene component does not alter the detection of the major gene nor the transmission probability estimates , which are close to the expected Mendelian values .
	manualset3
122216	6	404169	13	NULL	NULL	0	NULL	major gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the presence of a shared environmental effect in addition to a major gene component does not alter the detection of the major gene nor the transmission probability estimates , which are close to the expected Mendelian values .
	manualset3
122217	7	404169	13	NULL	NULL	0	NULL	transmission 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the presence of a shared environmental effect in addition to a major gene component does not alter the detection of the major gene nor the transmission probability estimates , which are close to the expected Mendelian values .
	manualset3
122218	8	404169	13	NULL	NULL	0	NULL	probability estimates 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the presence of a shared environmental effect in addition to a major gene component does not alter the detection of the major gene nor the transmission probability estimates , which are close to the expected Mendelian values .
	manualset3
122219	9	404169	13	NULL	NULL	0	NULL	Mendelian values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , the presence of a shared environmental effect in addition to a major gene component does not alter the detection of the major gene nor the transmission probability estimates , which are close to the expected Mendelian values .
	manualset3
122220	1	404170	13	NULL	NULL	0	NULL	GUVs	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , we observed in GUVs neither domain formation nor domain coalescence to be induced by the addition of detergents .
	manualset3
122221	2	404170	13	NULL	NULL	0	NULL	domain formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , we observed in GUVs neither domain formation nor domain coalescence to be induced by the addition of detergents .
	manualset3
122222	3	404170	13	NULL	NULL	0	NULL	domain coalescence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , we observed in GUVs neither domain formation nor domain coalescence to be induced by the addition of detergents .
	manualset3
122223	4	404170	13	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , we observed in GUVs neither domain formation nor domain coalescence to be induced by the addition of detergents .
	manualset3
122224	5	404170	13	NULL	NULL	0	NULL	detergents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , we observed in GUVs neither domain formation nor domain coalescence to be induced by the addition of detergents .
	manualset3
122225	1	404171	13	NULL	NULL	0	NULL	ketoconazole	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , we show that ketoconazole , a cytochrome P-450 inhibitor , hinders the wound closure induced by FCS in wounded 3T6 fibroblast cultures .
	manualset3
122226	2	404171	13	NULL	NULL	0	NULL	cytochrome P-450 inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , we show that ketoconazole , a cytochrome P-450 inhibitor , hinders the wound closure induced by FCS in wounded 3T6 fibroblast cultures .
	manualset3
122227	3	404171	13	NULL	NULL	0	NULL	wound closure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , we show that ketoconazole , a cytochrome P-450 inhibitor , hinders the wound closure induced by FCS in wounded 3T6 fibroblast cultures .
	manualset3
122228	4	404171	13	NULL	NULL	0	NULL	FCS	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , we show that ketoconazole , a cytochrome P-450 inhibitor , hinders the wound closure induced by FCS in wounded 3T6 fibroblast cultures .
	manualset3
122229	5	404171	13	NULL	NULL	0	NULL	3T6 fibroblast cultures 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , we show that ketoconazole , a cytochrome P-450 inhibitor , hinders the wound closure induced by FCS in wounded 3T6 fibroblast cultures .
	manualset3
122230	1	404172	13	NULL	NULL	0	NULL	angiotensin converting enzyme inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , when angiotensin converting enzyme inhibitors are already prescribed , nitrates can only be considered to improve symptoms in the case of persistence of dyspnoea .
	manualset3
122231	2	404172	13	NULL	NULL	0	NULL	nitrates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , when angiotensin converting enzyme inhibitors are already prescribed , nitrates can only be considered to improve symptoms in the case of persistence of dyspnoea .
	manualset3
122232	3	404172	13	NULL	NULL	0	NULL	symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , when angiotensin converting enzyme inhibitors are already prescribed , nitrates can only be considered to improve symptoms in the case of persistence of dyspnoea .
	manualset3
122233	4	404172	13	NULL	NULL	NULL	NULL	case	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On the other hand , when angiotensin converting enzyme inhibitors are already prescribed , nitrates can only be considered to improve symptoms in the case of persistence of dyspnoea .
	manualset3
122234	5	404172	13	NULL	NULL	0	NULL	persistence of dyspnoea	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , when angiotensin converting enzyme inhibitors are already prescribed , nitrates can only be considered to improve symptoms in the case of persistence of dyspnoea .
	manualset3
122252	1	404173	13	NULL	NULL	0	NULL	SOX9 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , while SOX9 expression immediately followed SRY expression in the B6 .
	manualset3
122253	2	404173	13	NULL	NULL	0	NULL	SRY expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , while SOX9 expression immediately followed SRY expression in the B6 .
	manualset3
122254	3	404173	13	NULL	NULL	0	NULL	B6	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , while SOX9 expression immediately followed SRY expression in the B6 .
	manualset3
122255	1	404174	13	NULL	NULL	0	NULL	plasma TXB2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , while plasma TXB2 was found elevated at 1 hour postoperatively in the control group , such a response to the surgical intervention was blocked and the plasma TXB2/6-keto prostaglandin ( PG ) F1a ratio was decreased in the OKY-046-treated group .
	manualset3
122256	2	404174	13	NULL	NULL	0	NULL	1 hour	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , while plasma TXB2 was found elevated at 1 hour postoperatively in the control group , such a response to the surgical intervention was blocked and the plasma TXB2/6-keto prostaglandin ( PG ) F1a ratio was decreased in the OKY-046-treated group .
	manualset3
122257	3	404174	13	NULL	NULL	0	NULL	control group 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , while plasma TXB2 was found elevated at 1 hour postoperatively in the control group , such a response to the surgical intervention was blocked and the plasma TXB2/6-keto prostaglandin ( PG ) F1a ratio was decreased in the OKY-046-treated group .
	manualset3
122258	4	404174	13	NULL	NULL	0	NULL	response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , while plasma TXB2 was found elevated at 1 hour postoperatively in the control group , such a response to the surgical intervention was blocked and the plasma TXB2/6-keto prostaglandin ( PG ) F1a ratio was decreased in the OKY-046-treated group .
	manualset3
122259	5	404174	13	NULL	NULL	0	NULL	surgical intervention 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , while plasma TXB2 was found elevated at 1 hour postoperatively in the control group , such a response to the surgical intervention was blocked and the plasma TXB2/6-keto prostaglandin ( PG ) F1a ratio was decreased in the OKY-046-treated group .
	manualset3
122260	6	404174	13	NULL	NULL	0	NULL	plasma TXB2/6-keto prostaglandin ( PG ) F1a ratio 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , while plasma TXB2 was found elevated at 1 hour postoperatively in the control group , such a response to the surgical intervention was blocked and the plasma TXB2/6-keto prostaglandin ( PG ) F1a ratio was decreased in the OKY-046-treated group .
	manualset3
122261	7	404174	13	NULL	NULL	0	NULL	OKY-046-treated group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , while plasma TXB2 was found elevated at 1 hour postoperatively in the control group , such a response to the surgical intervention was blocked and the plasma TXB2/6-keto prostaglandin ( PG ) F1a ratio was decreased in the OKY-046-treated group .
	manualset3
122262	1	404175	13	NULL	NULL	0	NULL	wild animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , wild or pasture fed animals such as the Herefords , Wild-boars and Touyuens had higher amounts of omega-3 fatty acids such as alpha-linolenic acid , icosapentaenoic acid and omega-6 fatty acids such as linoleic acid and arachidonic acid .
	manualset3
122263	2	404175	13	NULL	NULL	0	NULL	pasture fed animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , wild or pasture fed animals such as the Herefords , Wild-boars and Touyuens had higher amounts of omega-3 fatty acids such as alpha-linolenic acid , icosapentaenoic acid and omega-6 fatty acids such as linoleic acid and arachidonic acid .
	manualset3
122264	3	404175	13	NULL	NULL	0	NULL	Herefords	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , wild or pasture fed animals such as the Herefords , Wild-boars and Touyuens had higher amounts of omega-3 fatty acids such as alpha-linolenic acid , icosapentaenoic acid and omega-6 fatty acids such as linoleic acid and arachidonic acid .
	manualset3
122265	4	404175	13	NULL	NULL	0	NULL	Wild-boars	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , wild or pasture fed animals such as the Herefords , Wild-boars and Touyuens had higher amounts of omega-3 fatty acids such as alpha-linolenic acid , icosapentaenoic acid and omega-6 fatty acids such as linoleic acid and arachidonic acid .
	manualset3
122266	5	404175	13	NULL	NULL	0	NULL	Touyuens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , wild or pasture fed animals such as the Herefords , Wild-boars and Touyuens had higher amounts of omega-3 fatty acids such as alpha-linolenic acid , icosapentaenoic acid and omega-6 fatty acids such as linoleic acid and arachidonic acid .
	manualset3
122267	6	404175	13	NULL	NULL	0	NULL	amounts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , wild or pasture fed animals such as the Herefords , Wild-boars and Touyuens had higher amounts of omega-3 fatty acids such as alpha-linolenic acid , icosapentaenoic acid and omega-6 fatty acids such as linoleic acid and arachidonic acid .
	manualset3
122268	7	404175	13	NULL	NULL	0	NULL	omega-3 fatty acids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , wild or pasture fed animals such as the Herefords , Wild-boars and Touyuens had higher amounts of omega-3 fatty acids such as alpha-linolenic acid , icosapentaenoic acid and omega-6 fatty acids such as linoleic acid and arachidonic acid .
	manualset3
122269	8	404175	13	NULL	NULL	0	NULL	alpha-linolenic acid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , wild or pasture fed animals such as the Herefords , Wild-boars and Touyuens had higher amounts of omega-3 fatty acids such as alpha-linolenic acid , icosapentaenoic acid and omega-6 fatty acids such as linoleic acid and arachidonic acid .
	manualset3
122270	9	404175	13	NULL	NULL	0	NULL	icosapentaenoic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , wild or pasture fed animals such as the Herefords , Wild-boars and Touyuens had higher amounts of omega-3 fatty acids such as alpha-linolenic acid , icosapentaenoic acid and omega-6 fatty acids such as linoleic acid and arachidonic acid .
	manualset3
122271	10	404175	13	NULL	NULL	0	NULL	omega-6 fatty acids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , wild or pasture fed animals such as the Herefords , Wild-boars and Touyuens had higher amounts of omega-3 fatty acids such as alpha-linolenic acid , icosapentaenoic acid and omega-6 fatty acids such as linoleic acid and arachidonic acid .
	manualset3
122272	11	404175	13	NULL	NULL	0	NULL	linoleic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , wild or pasture fed animals such as the Herefords , Wild-boars and Touyuens had higher amounts of omega-3 fatty acids such as alpha-linolenic acid , icosapentaenoic acid and omega-6 fatty acids such as linoleic acid and arachidonic acid .
	manualset3
122273	12	404175	13	NULL	NULL	0	NULL	arachidonic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , wild or pasture fed animals such as the Herefords , Wild-boars and Touyuens had higher amounts of omega-3 fatty acids such as alpha-linolenic acid , icosapentaenoic acid and omega-6 fatty acids such as linoleic acid and arachidonic acid .
	manualset3
122274	1	404176	13	NULL	NULL	0	NULL	description	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A description of the key principles and concepts involved in telemedicine and a short historical overview of telemedicine 's evolution over the past century are followed by consideration of why empirical research into ` info-ethics ' and other deontological and legal issues relating to telemedicine is being necessarily catalysed by , amongst others , the European Commission .
	manualset3
122275	2	404176	13	NULL	NULL	NULL	NULL	key principles	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A description of the key principles and concepts involved in telemedicine and a short historical overview of telemedicine 's evolution over the past century are followed by consideration of why empirical research into ` info-ethics ' and other deontological and legal issues relating to telemedicine is being necessarily catalysed by , amongst others , the European Commission .
	manualset3
122276	3	404176	13	NULL	NULL	0	NULL	concepts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A description of the key principles and concepts involved in telemedicine and a short historical overview of telemedicine 's evolution over the past century are followed by consideration of why empirical research into ` info-ethics ' and other deontological and legal issues relating to telemedicine is being necessarily catalysed by , amongst others , the European Commission .
	manualset3
122277	4	404176	13	NULL	NULL	0	NULL	telemedicine 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A description of the key principles and concepts involved in telemedicine and a short historical overview of telemedicine 's evolution over the past century are followed by consideration of why empirical research into ` info-ethics ' and other deontological and legal issues relating to telemedicine is being necessarily catalysed by , amongst others , the European Commission .
	manualset3
122278	5	404176	13	NULL	NULL	0	NULL	overview	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A description of the key principles and concepts involved in telemedicine and a short historical overview of telemedicine 's evolution over the past century are followed by consideration of why empirical research into ` info-ethics ' and other deontological and legal issues relating to telemedicine is being necessarily catalysed by , amongst others , the European Commission .
	manualset3
122279	6	404176	13	NULL	NULL	0	NULL	telemedicine 's evolution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A description of the key principles and concepts involved in telemedicine and a short historical overview of telemedicine 's evolution over the past century are followed by consideration of why empirical research into ` info-ethics ' and other deontological and legal issues relating to telemedicine is being necessarily catalysed by , amongst others , the European Commission .
	manualset3
122280	7	404176	13	NULL	NULL	0	NULL	past century 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A description of the key principles and concepts involved in telemedicine and a short historical overview of telemedicine 's evolution over the past century are followed by consideration of why empirical research into ` info-ethics ' and other deontological and legal issues relating to telemedicine is being necessarily catalysed by , amongst others , the European Commission .
	manualset3
122281	8	404176	13	NULL	NULL	0	NULL	consideration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A description of the key principles and concepts involved in telemedicine and a short historical overview of telemedicine 's evolution over the past century are followed by consideration of why empirical research into ` info-ethics ' and other deontological and legal issues relating to telemedicine is being necessarily catalysed by , amongst others , the European Commission .
	manualset3
122282	9	404176	13	NULL	NULL	0	NULL	empirical research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A description of the key principles and concepts involved in telemedicine and a short historical overview of telemedicine 's evolution over the past century are followed by consideration of why empirical research into ` info-ethics ' and other deontological and legal issues relating to telemedicine is being necessarily catalysed by , amongst others , the European Commission .
	manualset3
122283	10	404176	13	NULL	NULL	0	NULL	deontological issues	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A description of the key principles and concepts involved in telemedicine and a short historical overview of telemedicine 's evolution over the past century are followed by consideration of why empirical research into ` info-ethics ' and other deontological and legal issues relating to telemedicine is being necessarily catalysed by , amongst others , the European Commission .
	manualset3
122284	11	404176	13	NULL	NULL	0	NULL	legal issues	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A description of the key principles and concepts involved in telemedicine and a short historical overview of telemedicine 's evolution over the past century are followed by consideration of why empirical research into ` info-ethics ' and other deontological and legal issues relating to telemedicine is being necessarily catalysed by , amongst others , the European Commission .
	manualset3
122285	12	404176	13	NULL	NULL	0	NULL	telemedicine	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A description of the key principles and concepts involved in telemedicine and a short historical overview of telemedicine 's evolution over the past century are followed by consideration of why empirical research into ` info-ethics ' and other deontological and legal issues relating to telemedicine is being necessarily catalysed by , amongst others , the European Commission .
	manualset3
122286	13	404176	13	NULL	NULL	0	NULL	European Commission 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A description of the key principles and concepts involved in telemedicine and a short historical overview of telemedicine 's evolution over the past century are followed by consideration of why empirical research into ` info-ethics ' and other deontological and legal issues relating to telemedicine is being necessarily catalysed by , amongst others , the European Commission .
	manualset3
122287	1	404177	13	NULL	NULL	0	NULL	 hyperaemic perfusion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand hyperaemic perfusion is reduced , but is not explained by A2AR density .
	manualset3
122288	2	404177	13	NULL	NULL	0	NULL	A2AR density	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand hyperaemic perfusion is reduced , but is not explained by A2AR density .
	manualset3
122289	1	404178	13	NULL	NULL	0	NULL	cadmium sulfide nanoparticles	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand the cadmium sulfide nanoparticles , grown into the cyclic olefin copolymer matrix , exhibit narrower emission spectra .
	manualset3
122290	2	404178	13	NULL	NULL	0	NULL	 cyclic olefin copolymer matrix	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand the cadmium sulfide nanoparticles , grown into the cyclic olefin copolymer matrix , exhibit narrower emission spectra .
	manualset3
122291	3	404178	13	NULL	NULL	0	NULL	emission spectra 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand the cadmium sulfide nanoparticles , grown into the cyclic olefin copolymer matrix , exhibit narrower emission spectra .
	manualset3
122292	1	404179	13	NULL	NULL	0	NULL	no-pair approximation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the practical side , it is shown that , under the no-pair approximation , relativistic explicitly correlated wave function methods can be made completely parallel to the nonrelativistic counterparts , as demonstrated explicitly for MP2-F12 .
	manualset3
122293	2	404179	13	NULL	NULL	0	NULL	wave function methods	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the practical side , it is shown that , under the no-pair approximation , relativistic explicitly correlated wave function methods can be made completely parallel to the nonrelativistic counterparts , as demonstrated explicitly for MP2-F12 .
	manualset3
122294	3	404179	13	NULL	NULL	0	NULL	nonrelativistic counterparts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the practical side , it is shown that , under the no-pair approximation , relativistic explicitly correlated wave function methods can be made completely parallel to the nonrelativistic counterparts , as demonstrated explicitly for MP2-F12 .
	manualset3
122295	4	404179	13	NULL	NULL	0	NULL	MP2-F12	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	On the practical side , it is shown that , under the no-pair approximation , relativistic explicitly correlated wave function methods can be made completely parallel to the nonrelativistic counterparts , as demonstrated explicitly for MP2-F12 .
	manualset3
122296	1	404180	13	NULL	NULL	0	NULL	predictive recognition	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the predictive recognition of signal peptide sequences .
	manualset3
122297	2	404180	13	NULL	NULL	0	NULL	signal peptide sequences	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	On the predictive recognition of signal peptide sequences .
	manualset3
122359	1	404181	13	NULL	NULL	0	NULL	recovery 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the recovery of protozoa and eggs of some species of helminths in human feces .
	manualset3
122360	2	404181	13	NULL	NULL	0	NULL	protozoa	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On the recovery of protozoa and eggs of some species of helminths in human feces .
	manualset3
122361	3	404181	13	NULL	NULL	0	NULL	eggs 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	On the recovery of protozoa and eggs of some species of helminths in human feces .
	manualset3
122362	4	404181	13	NULL	NULL	0	NULL	species of helminths	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On the recovery of protozoa and eggs of some species of helminths in human feces .
	manualset3
122363	5	404181	13	NULL	NULL	0	NULL	human feces	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the recovery of protozoa and eggs of some species of helminths in human feces .
	manualset3
122364	1	404182	13	NULL	NULL	0	NULL	sad mood	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the sad mood induction night , participants in both groups had shorter SOL and increased REM density when compared to the baseline nights .
	manualset3
122365	2	404182	13	NULL	NULL	0	NULL	induction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the sad mood induction night , participants in both groups had shorter SOL and increased REM density when compared to the baseline nights .
	manualset3
122366	3	404182	13	NULL	NULL	0	NULL	night	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	On the sad mood induction night , participants in both groups had shorter SOL and increased REM density when compared to the baseline nights .
	manualset3
122367	4	404182	13	NULL	NULL	0	NULL	participants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On the sad mood induction night , participants in both groups had shorter SOL and increased REM density when compared to the baseline nights .
	manualset3
122368	5	404182	13	NULL	NULL	0	NULL	groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On the sad mood induction night , participants in both groups had shorter SOL and increased REM density when compared to the baseline nights .
	manualset3
122369	6	404182	13	NULL	NULL	0	NULL	shorter SOL	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the sad mood induction night , participants in both groups had shorter SOL and increased REM density when compared to the baseline nights .
	manualset3
122370	7	404182	13	NULL	NULL	0	NULL	REM density 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the sad mood induction night , participants in both groups had shorter SOL and increased REM density when compared to the baseline nights .
	manualset3
122371	8	404182	13	NULL	NULL	0	NULL	baseline	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the sad mood induction night , participants in both groups had shorter SOL and increased REM density when compared to the baseline nights .
	manualset3
122372	9	404182	13	NULL	NULL	0	NULL	nights	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	On the sad mood induction night , participants in both groups had shorter SOL and increased REM density when compared to the baseline nights .
	manualset3
122373	1	404183	13	NULL	NULL	0	NULL	tenth day	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	On the tenth day after admission , severe dysphagia , dysphonia , irritative cough and further enlargement of the neck mass developed .
	manualset3
122374	2	404183	13	NULL	NULL	0	NULL	admission 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the tenth day after admission , severe dysphagia , dysphonia , irritative cough and further enlargement of the neck mass developed .
	manualset3
122375	3	404183	13	NULL	NULL	0	NULL	severe dysphagia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the tenth day after admission , severe dysphagia , dysphonia , irritative cough and further enlargement of the neck mass developed .
	manualset3
122376	4	404183	13	NULL	NULL	0	NULL	dysphonia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the tenth day after admission , severe dysphagia , dysphonia , irritative cough and further enlargement of the neck mass developed .
	manualset3
122377	5	404183	13	NULL	NULL	0	NULL	irritative cough	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the tenth day after admission , severe dysphagia , dysphonia , irritative cough and further enlargement of the neck mass developed .
	manualset3
122378	6	404183	13	NULL	NULL	0	NULL	enlargement of the neck mass	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the tenth day after admission , severe dysphagia , dysphonia , irritative cough and further enlargement of the neck mass developed .
	manualset3
122379	1	404184	13	NULL	NULL	0	NULL	third day	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	On the third day , pulmonary blood flow scintigraphy was performed because of progression of his dyspnea , and showed multiple defects indicating widespread thrombi in the peripheral pulmonary arteries .
	manualset3
122380	2	404184	13	NULL	NULL	0	NULL	pulmonary blood flow scintigraphy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	On the third day , pulmonary blood flow scintigraphy was performed because of progression of his dyspnea , and showed multiple defects indicating widespread thrombi in the peripheral pulmonary arteries .
	manualset3
122381	3	404184	13	NULL	NULL	0	NULL	progression 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the third day , pulmonary blood flow scintigraphy was performed because of progression of his dyspnea , and showed multiple defects indicating widespread thrombi in the peripheral pulmonary arteries .
	manualset3
122382	4	404184	13	NULL	NULL	0	NULL	dyspnea	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the third day , pulmonary blood flow scintigraphy was performed because of progression of his dyspnea , and showed multiple defects indicating widespread thrombi in the peripheral pulmonary arteries .
	manualset3
122383	5	404184	13	NULL	NULL	0	NULL	multiple defects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the third day , pulmonary blood flow scintigraphy was performed because of progression of his dyspnea , and showed multiple defects indicating widespread thrombi in the peripheral pulmonary arteries .
	manualset3
122384	6	404184	13	NULL	NULL	0	NULL	thrombi	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the third day , pulmonary blood flow scintigraphy was performed because of progression of his dyspnea , and showed multiple defects indicating widespread thrombi in the peripheral pulmonary arteries .
	manualset3
122385	7	404184	13	NULL	NULL	0	NULL	peripheral pulmonary arteries 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	On the third day , pulmonary blood flow scintigraphy was performed because of progression of his dyspnea , and showed multiple defects indicating widespread thrombi in the peripheral pulmonary arteries .
	manualset3
122386	1	404185	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A descriptive study has documented what is felt to be a precise estimate of the prevalence of epilepsy in 1973 in the school-age population of Clay County , Kentucky , a rural Appalachian county .
	manualset3
122387	2	404185	13	NULL	NULL	NULL	NULL	precise estimate	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A descriptive study has documented what is felt to be a precise estimate of the prevalence of epilepsy in 1973 in the school-age population of Clay County , Kentucky , a rural Appalachian county .
	manualset3
122388	3	404185	13	NULL	NULL	0	NULL	prevalence of epilepsy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A descriptive study has documented what is felt to be a precise estimate of the prevalence of epilepsy in 1973 in the school-age population of Clay County , Kentucky , a rural Appalachian county .
	manualset3
122389	4	404185	13	NULL	NULL	0	NULL	1973	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	A descriptive study has documented what is felt to be a precise estimate of the prevalence of epilepsy in 1973 in the school-age population of Clay County , Kentucky , a rural Appalachian county .
	manualset3
122390	5	404185	13	NULL	NULL	0	NULL	school-age population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A descriptive study has documented what is felt to be a precise estimate of the prevalence of epilepsy in 1973 in the school-age population of Clay County , Kentucky , a rural Appalachian county .
	manualset3
122391	6	404185	13	NULL	NULL	0	NULL	Clay County	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A descriptive study has documented what is felt to be a precise estimate of the prevalence of epilepsy in 1973 in the school-age population of Clay County , Kentucky , a rural Appalachian county .
	manualset3
122392	7	404185	13	NULL	NULL	0	NULL	Kentucky	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A descriptive study has documented what is felt to be a precise estimate of the prevalence of epilepsy in 1973 in the school-age population of Clay County , Kentucky , a rural Appalachian county .
	manualset3
122393	8	404185	13	NULL	NULL	0	NULL	rural Appalachian county	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A descriptive study has documented what is felt to be a precise estimate of the prevalence of epilepsy in 1973 in the school-age population of Clay County , Kentucky , a rural Appalachian county .
	manualset3
122394	1	404186	13	NULL	NULL	0	NULL	ultrastructure of ependymomas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the ultrastructure of ependymomas -- a semiquantitative analysis of diagnostic criteria in 21 cases with special reference to glycogen as a marker .
	manualset3
122395	2	404186	13	NULL	NULL	0	NULL	semiquantitative analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the ultrastructure of ependymomas -- a semiquantitative analysis of diagnostic criteria in 21 cases with special reference to glycogen as a marker .
	manualset3
122396	3	404186	13	NULL	NULL	0	NULL	diagnostic criteria	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the ultrastructure of ependymomas -- a semiquantitative analysis of diagnostic criteria in 21 cases with special reference to glycogen as a marker .
	manualset3
122397	4	404186	13	NULL	NULL	0	NULL	21 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On the ultrastructure of ependymomas -- a semiquantitative analysis of diagnostic criteria in 21 cases with special reference to glycogen as a marker .
	manualset3
122398	5	404186	13	NULL	NULL	0	NULL	reference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the ultrastructure of ependymomas -- a semiquantitative analysis of diagnostic criteria in 21 cases with special reference to glycogen as a marker .
	manualset3
122399	6	404186	13	NULL	NULL	0	NULL	 glycogen	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the ultrastructure of ependymomas -- a semiquantitative analysis of diagnostic criteria in 21 cases with special reference to glycogen as a marker .
	manualset3
122400	7	404186	13	NULL	NULL	0	NULL	marker	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the ultrastructure of ependymomas -- a semiquantitative analysis of diagnostic criteria in 21 cases with special reference to glycogen as a marker .
	manualset3
122401	1	404187	13	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the use of methods , abstinence , breastfeeding and use of condoms recorded 42.8 % , 22 % and 40.3 % respectively .
	manualset3
122402	2	404187	13	NULL	NULL	0	NULL	methods	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the use of methods , abstinence , breastfeeding and use of condoms recorded 42.8 % , 22 % and 40.3 % respectively .
	manualset3
122403	3	404187	13	NULL	NULL	0	NULL	abstinence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the use of methods , abstinence , breastfeeding and use of condoms recorded 42.8 % , 22 % and 40.3 % respectively .
	manualset3
122404	4	404187	13	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the use of methods , abstinence , breastfeeding and use of condoms recorded 42.8 % , 22 % and 40.3 % respectively .
	manualset3
122405	5	404187	13	NULL	NULL	0	NULL	condoms	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	On the use of methods , abstinence , breastfeeding and use of condoms recorded 42.8 % , 22 % and 40.3 % respectively .
	manualset3
122406	6	404187	13	NULL	NULL	0	NULL	42.8 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the use of methods , abstinence , breastfeeding and use of condoms recorded 42.8 % , 22 % and 40.3 % respectively .
	manualset3
122407	7	404187	13	NULL	NULL	0	NULL	22 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the use of methods , abstinence , breastfeeding and use of condoms recorded 42.8 % , 22 % and 40.3 % respectively .
	manualset3
122408	8	404187	13	NULL	NULL	0	NULL	40.3 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the use of methods , abstinence , breastfeeding and use of condoms recorded 42.8 % , 22 % and 40.3 % respectively .
	manualset3
122432	1	404188	13	NULL	NULL	0	NULL	way	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On this way a network of care units could be established within the leading regional institutions , which would further the elaboration of unitary directives for the examination and treatment of patients .
	manualset3
122433	2	404188	13	NULL	NULL	0	NULL	network	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On this way a network of care units could be established within the leading regional institutions , which would further the elaboration of unitary directives for the examination and treatment of patients .
	manualset3
122434	3	404188	13	NULL	NULL	0	NULL	care units	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	On this way a network of care units could be established within the leading regional institutions , which would further the elaboration of unitary directives for the examination and treatment of patients .
	manualset3
122435	4	404188	13	NULL	NULL	0	NULL	regional institutions	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	On this way a network of care units could be established within the leading regional institutions , which would further the elaboration of unitary directives for the examination and treatment of patients .
	manualset3
122446	5	404188	13	NULL	NULL	0	NULL	elaboration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On this way a network of care units could be established within the leading regional institutions , which would further the elaboration of unitary directives for the examination and treatment of patients .
	manualset3
122447	6	404188	13	NULL	NULL	0	NULL	unitary directives 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On this way a network of care units could be established within the leading regional institutions , which would further the elaboration of unitary directives for the examination and treatment of patients .
	manualset3
122448	7	404188	13	NULL	NULL	0	NULL	examination 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	On this way a network of care units could be established within the leading regional institutions , which would further the elaboration of unitary directives for the examination and treatment of patients .
	manualset3
122449	8	404188	13	NULL	NULL	NULL	NULL	treatment 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On this way a network of care units could be established within the leading regional institutions , which would further the elaboration of unitary directives for the examination and treatment of patients .
	manualset3
122450	9	404188	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On this way a network of care units could be established within the leading regional institutions , which would further the elaboration of unitary directives for the examination and treatment of patients .
	manualset3
122451	1	404189	13	NULL	NULL	0	NULL	fruit fly	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Once again the humble fruit fly is providing a genetic framework for understanding complex regulatory systems which have been conserved during evolution .
	manualset3
122452	2	404189	13	NULL	NULL	0	NULL	genetic framework	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Once again the humble fruit fly is providing a genetic framework for understanding complex regulatory systems which have been conserved during evolution .
	manualset3
122453	3	404189	13	NULL	NULL	0	NULL	complex regulatory systems	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Once again the humble fruit fly is providing a genetic framework for understanding complex regulatory systems which have been conserved during evolution .
	manualset3
122454	4	404189	13	NULL	NULL	0	NULL	evolution 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Once again the humble fruit fly is providing a genetic framework for understanding complex regulatory systems which have been conserved during evolution .
	manualset3
122455	1	404190	13	NULL	NULL	0	NULL	cell	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Once enriched/preconcentrated inside the cell , they are released by removal of the electric field and via an interface with an electrospray emitter are submitted to online mass spectrometric analysis .
	manualset3
122456	2	404190	13	NULL	NULL	0	NULL	removal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Once enriched/preconcentrated inside the cell , they are released by removal of the electric field and via an interface with an electrospray emitter are submitted to online mass spectrometric analysis .
	manualset3
122457	3	404190	13	NULL	NULL	0	NULL	electric field 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Once enriched/preconcentrated inside the cell , they are released by removal of the electric field and via an interface with an electrospray emitter are submitted to online mass spectrometric analysis .
	manualset3
122458	4	404190	13	NULL	NULL	0	NULL	interface	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Once enriched/preconcentrated inside the cell , they are released by removal of the electric field and via an interface with an electrospray emitter are submitted to online mass spectrometric analysis .
	manualset3
122459	5	404190	13	NULL	NULL	0	NULL	electrospray emitter	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Once enriched/preconcentrated inside the cell , they are released by removal of the electric field and via an interface with an electrospray emitter are submitted to online mass spectrometric analysis .
	manualset3
122460	6	404190	13	NULL	NULL	0	NULL	online mass spectrometric analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Once enriched/preconcentrated inside the cell , they are released by removal of the electric field and via an interface with an electrospray emitter are submitted to online mass spectrometric analysis .
	manualset3
122461	1	404191	13	NULL	NULL	0	NULL	pp65 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Once made , pp65 showed the same characteristics as naturally produced protein and was stable for several days in astrocytoma cells , as it is during HCMV replication in fibroblasts .
	manualset3
122462	2	404191	13	NULL	NULL	0	NULL	characteristics	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Once made , pp65 showed the same characteristics as naturally produced protein and was stable for several days in astrocytoma cells , as it is during HCMV replication in fibroblasts .
	manualset3
122463	3	404191	13	NULL	NULL	0	NULL	protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Once made , pp65 showed the same characteristics as naturally produced protein and was stable for several days in astrocytoma cells , as it is during HCMV replication in fibroblasts .
	manualset3
122464	4	404191	13	NULL	NULL	0	NULL	several days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Once made , pp65 showed the same characteristics as naturally produced protein and was stable for several days in astrocytoma cells , as it is during HCMV replication in fibroblasts .
	manualset3
122465	5	404191	13	NULL	NULL	0	NULL	astrocytoma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Once made , pp65 showed the same characteristics as naturally produced protein and was stable for several days in astrocytoma cells , as it is during HCMV replication in fibroblasts .
	manualset3
122466	6	404191	13	NULL	NULL	0	NULL	HCMV replication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Once made , pp65 showed the same characteristics as naturally produced protein and was stable for several days in astrocytoma cells , as it is during HCMV replication in fibroblasts .
	manualset3
122467	7	404191	13	NULL	NULL	0	NULL	fibroblasts 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Once made , pp65 showed the same characteristics as naturally produced protein and was stable for several days in astrocytoma cells , as it is during HCMV replication in fibroblasts .
	manualset3
122468	1	404192	13	NULL	NULL	0	NULL	aging	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Once regarded as an inevitable part of aging , osteoporosis and fracture risk are now recognized as preventable and treatable .
	manualset3
122469	2	404192	13	NULL	NULL	0	NULL	osteoporosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Once regarded as an inevitable part of aging , osteoporosis and fracture risk are now recognized as preventable and treatable .
	manualset3
122470	3	404192	13	NULL	NULL	0	NULL	fracture risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Once regarded as an inevitable part of aging , osteoporosis and fracture risk are now recognized as preventable and treatable .
	manualset3
122471	1	404193	13	NULL	NULL	0	NULL	immunosuppressed states	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Once seen primarily in severely immunosuppressed states including lymphoma , solid organ malignancies , and organ transplant recipients , PML became an AIDS-defining illness in the 1980s .
	manualset3
122472	2	404193	13	NULL	NULL	0	NULL	lymphoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Once seen primarily in severely immunosuppressed states including lymphoma , solid organ malignancies , and organ transplant recipients , PML became an AIDS-defining illness in the 1980s .
	manualset3
122474	3	404193	13	NULL	NULL	0	NULL	solid organ malignancies 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Once seen primarily in severely immunosuppressed states including lymphoma , solid organ malignancies , and organ transplant recipients , PML became an AIDS-defining illness in the 1980s .
	manualset3
122476	4	404193	13	NULL	NULL	0	NULL	organ transplant recipients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Once seen primarily in severely immunosuppressed states including lymphoma , solid organ malignancies , and organ transplant recipients , PML became an AIDS-defining illness in the 1980s .
	manualset3
122477	5	404193	13	NULL	NULL	0	NULL	PML 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Once seen primarily in severely immunosuppressed states including lymphoma , solid organ malignancies , and organ transplant recipients , PML became an AIDS-defining illness in the 1980s .
	manualset3
122478	6	404193	13	NULL	NULL	0	NULL	AIDS-defining illness 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Once seen primarily in severely immunosuppressed states including lymphoma , solid organ malignancies , and organ transplant recipients , PML became an AIDS-defining illness in the 1980s .
	manualset3
122479	7	404193	13	NULL	NULL	0	NULL	1980s 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Once seen primarily in severely immunosuppressed states including lymphoma , solid organ malignancies , and organ transplant recipients , PML became an AIDS-defining illness in the 1980s .
	manualset3
122480	1	404194	13	NULL	NULL	NULL	NULL	diagnosis	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Once the diagnosis is confirmed , definitive surgery is mandatory because recurrence and metastatic disease have a low 5-year survival rate .
	manualset3
122481	2	404194	13	NULL	NULL	0	NULL	definitive surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Once the diagnosis is confirmed , definitive surgery is mandatory because recurrence and metastatic disease have a low 5-year survival rate .
	manualset3
122482	3	404194	13	NULL	NULL	0	NULL	recurrence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Once the diagnosis is confirmed , definitive surgery is mandatory because recurrence and metastatic disease have a low 5-year survival rate .
	manualset3
122483	4	404194	13	NULL	NULL	0	NULL	metastatic disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Once the diagnosis is confirmed , definitive surgery is mandatory because recurrence and metastatic disease have a low 5-year survival rate .
	manualset3
122484	5	404194	13	NULL	NULL	0	NULL	5-year	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Once the diagnosis is confirmed , definitive surgery is mandatory because recurrence and metastatic disease have a low 5-year survival rate .
	manualset3
122485	6	404194	13	NULL	NULL	0	NULL	survival rate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Once the diagnosis is confirmed , definitive surgery is mandatory because recurrence and metastatic disease have a low 5-year survival rate .
	manualset3
122538	1	404195	13	NULL	NULL	0	NULL	descriptive study	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A descriptive study of eleven healthy preterm infants was conducted in which cardiorespiratory ( heart and respiratory rates , oxygen saturation ) , thermal ( abdominal , toe and tympanic temperatures ) and state behavior responses to two hours of paternal skin-to-skin contact within the first 17 hours of birth in Colombia , South America were evaluated .
	manualset3
122539	2	404195	13	NULL	NULL	0	NULL	eleven healthy preterm infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A descriptive study of eleven healthy preterm infants was conducted in which cardiorespiratory ( heart and respiratory rates , oxygen saturation ) , thermal ( abdominal , toe and tympanic temperatures ) and state behavior responses to two hours of paternal skin-to-skin contact within the first 17 hours of birth in Colombia , South America were evaluated .
	manualset3
122540	3	404195	13	NULL	NULL	0	NULL	heart rates 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A descriptive study of eleven healthy preterm infants was conducted in which cardiorespiratory ( heart and respiratory rates , oxygen saturation ) , thermal ( abdominal , toe and tympanic temperatures ) and state behavior responses to two hours of paternal skin-to-skin contact within the first 17 hours of birth in Colombia , South America were evaluated .
	manualset3
122541	4	404195	13	NULL	NULL	0	NULL	respiratory rates 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A descriptive study of eleven healthy preterm infants was conducted in which cardiorespiratory ( heart and respiratory rates , oxygen saturation ) , thermal ( abdominal , toe and tympanic temperatures ) and state behavior responses to two hours of paternal skin-to-skin contact within the first 17 hours of birth in Colombia , South America were evaluated .
	manualset3
122542	5	404195	13	NULL	NULL	0	NULL	oxygen saturation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A descriptive study of eleven healthy preterm infants was conducted in which cardiorespiratory ( heart and respiratory rates , oxygen saturation ) , thermal ( abdominal , toe and tympanic temperatures ) and state behavior responses to two hours of paternal skin-to-skin contact within the first 17 hours of birth in Colombia , South America were evaluated .
	manualset3
122543	6	404195	13	NULL	NULL	0	NULL	abdominal temperatures 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A descriptive study of eleven healthy preterm infants was conducted in which cardiorespiratory ( heart and respiratory rates , oxygen saturation ) , thermal ( abdominal , toe and tympanic temperatures ) and state behavior responses to two hours of paternal skin-to-skin contact within the first 17 hours of birth in Colombia , South America were evaluated .
	manualset3
122544	7	404195	13	NULL	NULL	0	NULL	toe temperatures 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A descriptive study of eleven healthy preterm infants was conducted in which cardiorespiratory ( heart and respiratory rates , oxygen saturation ) , thermal ( abdominal , toe and tympanic temperatures ) and state behavior responses to two hours of paternal skin-to-skin contact within the first 17 hours of birth in Colombia , South America were evaluated .
	manualset3
122545	8	404195	13	NULL	NULL	0	NULL	tympanic temperatures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A descriptive study of eleven healthy preterm infants was conducted in which cardiorespiratory ( heart and respiratory rates , oxygen saturation ) , thermal ( abdominal , toe and tympanic temperatures ) and state behavior responses to two hours of paternal skin-to-skin contact within the first 17 hours of birth in Colombia , South America were evaluated .
	manualset3
122546	9	404195	13	NULL	NULL	0	NULL	state behavior responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A descriptive study of eleven healthy preterm infants was conducted in which cardiorespiratory ( heart and respiratory rates , oxygen saturation ) , thermal ( abdominal , toe and tympanic temperatures ) and state behavior responses to two hours of paternal skin-to-skin contact within the first 17 hours of birth in Colombia , South America were evaluated .
	manualset3
122547	10	404195	13	NULL	NULL	0	NULL	two hours 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A descriptive study of eleven healthy preterm infants was conducted in which cardiorespiratory ( heart and respiratory rates , oxygen saturation ) , thermal ( abdominal , toe and tympanic temperatures ) and state behavior responses to two hours of paternal skin-to-skin contact within the first 17 hours of birth in Colombia , South America were evaluated .
	manualset3
122548	11	404195	13	NULL	NULL	0	NULL	paternal skin-to-skin contact	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A descriptive study of eleven healthy preterm infants was conducted in which cardiorespiratory ( heart and respiratory rates , oxygen saturation ) , thermal ( abdominal , toe and tympanic temperatures ) and state behavior responses to two hours of paternal skin-to-skin contact within the first 17 hours of birth in Colombia , South America were evaluated .
	manualset3
122549	12	404195	13	NULL	NULL	0	NULL	first 17 hours 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A descriptive study of eleven healthy preterm infants was conducted in which cardiorespiratory ( heart and respiratory rates , oxygen saturation ) , thermal ( abdominal , toe and tympanic temperatures ) and state behavior responses to two hours of paternal skin-to-skin contact within the first 17 hours of birth in Colombia , South America were evaluated .
	manualset3
122550	13	404195	13	NULL	NULL	0	NULL	birth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A descriptive study of eleven healthy preterm infants was conducted in which cardiorespiratory ( heart and respiratory rates , oxygen saturation ) , thermal ( abdominal , toe and tympanic temperatures ) and state behavior responses to two hours of paternal skin-to-skin contact within the first 17 hours of birth in Colombia , South America were evaluated .
	manualset3
122551	14	404195	13	NULL	NULL	0	NULL	Colombia	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A descriptive study of eleven healthy preterm infants was conducted in which cardiorespiratory ( heart and respiratory rates , oxygen saturation ) , thermal ( abdominal , toe and tympanic temperatures ) and state behavior responses to two hours of paternal skin-to-skin contact within the first 17 hours of birth in Colombia , South America were evaluated .
	manualset3
122552	15	404195	13	NULL	NULL	0	NULL	South America	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A descriptive study of eleven healthy preterm infants was conducted in which cardiorespiratory ( heart and respiratory rates , oxygen saturation ) , thermal ( abdominal , toe and tympanic temperatures ) and state behavior responses to two hours of paternal skin-to-skin contact within the first 17 hours of birth in Colombia , South America were evaluated .
	manualset3
122553	1	404196	13	NULL	NULL	0	NULL	lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Once the lymphocytes are transformed no demand of purines is necessary and the uptake and metabolism is switched off .
	manualset3
122554	2	404196	13	NULL	NULL	0	NULL	demand	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Once the lymphocytes are transformed no demand of purines is necessary and the uptake and metabolism is switched off .
	manualset3
122555	3	404196	13	NULL	NULL	0	NULL	purines 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Once the lymphocytes are transformed no demand of purines is necessary and the uptake and metabolism is switched off .
	manualset3
122556	4	404196	13	NULL	NULL	0	NULL	uptake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Once the lymphocytes are transformed no demand of purines is necessary and the uptake and metabolism is switched off .
	manualset3
122557	5	404196	13	NULL	NULL	0	NULL	metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Once the lymphocytes are transformed no demand of purines is necessary and the uptake and metabolism is switched off .
	manualset3
122558	1	404197	13	NULL	NULL	0	NULL	droplet 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Once they have diffused into the droplet , the I ( 2 ) molecules sometimes iodinate accessible tyrosines at ortho positions .
	manualset3
122559	2	404197	13	NULL	NULL	0	NULL	I ( 2 ) molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Once they have diffused into the droplet , the I ( 2 ) molecules sometimes iodinate accessible tyrosines at ortho positions .
	manualset3
122560	3	404197	13	NULL	NULL	0	NULL	tyrosines	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Once they have diffused into the droplet , the I ( 2 ) molecules sometimes iodinate accessible tyrosines at ortho positions .
	manualset3
122561	4	404197	13	NULL	NULL	NULL	NULL	ortho positions	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Once they have diffused into the droplet , the I ( 2 ) molecules sometimes iodinate accessible tyrosines at ortho positions .
	manualset3
125243	5	404197	13	NULL	NULL	0	NULL	iodinate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Once they have diffused into the droplet , the I ( 2 ) molecules sometimes iodinate accessible tyrosines at ortho positions .
	manualset3
122562	1	404198	13	NULL	NULL	0	NULL	lever-pressing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Once training was complete , lever-pressing was extinguished in the absence of either sucrose or CS presentation .
	manualset3
122563	2	404198	13	NULL	NULL	0	NULL	absence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Once training was complete , lever-pressing was extinguished in the absence of either sucrose or CS presentation .
	manualset3
122564	3	404198	13	NULL	NULL	0	NULL	sucrose 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Once training was complete , lever-pressing was extinguished in the absence of either sucrose or CS presentation .
	manualset3
122565	4	404198	13	NULL	NULL	0	NULL	CS presentation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Once training was complete , lever-pressing was extinguished in the absence of either sucrose or CS presentation .
	manualset3
122566	1	404199	13	NULL	NULL	0	NULL	Oncogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Oncogenesis is the consequence of a series of genetic alterations that allow unrestrained cellular growth , tissue invasion , and eventual metastases .
	manualset3
122567	2	404199	13	NULL	NULL	0	NULL	consequence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Oncogenesis is the consequence of a series of genetic alterations that allow unrestrained cellular growth , tissue invasion , and eventual metastases .
	manualset3
122568	3	404199	13	NULL	NULL	0	NULL	series of genetic alterations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Oncogenesis is the consequence of a series of genetic alterations that allow unrestrained cellular growth , tissue invasion , and eventual metastases .
	manualset3
122569	4	404199	13	NULL	NULL	0	NULL	unrestrained cellular growth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Oncogenesis is the consequence of a series of genetic alterations that allow unrestrained cellular growth , tissue invasion , and eventual metastases .
	manualset3
122570	5	404199	13	NULL	NULL	0	NULL	tissue invasion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Oncogenesis is the consequence of a series of genetic alterations that allow unrestrained cellular growth , tissue invasion , and eventual metastases .
	manualset3
122571	6	404199	13	NULL	NULL	0	NULL	eventual metastases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Oncogenesis is the consequence of a series of genetic alterations that allow unrestrained cellular growth , tissue invasion , and eventual metastases .
	manualset3
122572	1	404200	13	NULL	NULL	0	NULL	Oncogenic tyrosine kinases 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Oncogenic tyrosine kinases target Dok-1 for ubiquitin-mediated proteasomal degradation to promote cell transformation .
	manualset3
122573	2	404200	13	NULL	NULL	0	NULL	target	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Oncogenic tyrosine kinases target Dok-1 for ubiquitin-mediated proteasomal degradation to promote cell transformation .
	manualset3
122574	3	404200	13	NULL	NULL	0	NULL	Dok-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Oncogenic tyrosine kinases target Dok-1 for ubiquitin-mediated proteasomal degradation to promote cell transformation .
	manualset3
122575	4	404200	13	NULL	NULL	0	NULL	ubiquitin-mediated proteasomal degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Oncogenic tyrosine kinases target Dok-1 for ubiquitin-mediated proteasomal degradation to promote cell transformation .
	manualset3
122576	5	404200	13	NULL	NULL	0	NULL	cell transformation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Oncogenic tyrosine kinases target Dok-1 for ubiquitin-mediated proteasomal degradation to promote cell transformation .
	manualset3
122577	1	404201	13	NULL	NULL	0	NULL	One-third 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One-third of pregnant women reported being screened for IPV .
	manualset3
122578	2	404201	13	NULL	NULL	0	NULL	pregnant women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One-third of pregnant women reported being screened for IPV .
	manualset3
122579	3	404201	13	NULL	NULL	0	NULL	IPV	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One-third of pregnant women reported being screened for IPV .
	manualset3
122580	1	404202	13	NULL	NULL	0	NULL	clinical study	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A detailed clinical and autoptic study of a case of alcoholic beri-beri is presented .
	manualset3
122581	2	404202	13	NULL	NULL	0	NULL	autoptic study	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A detailed clinical and autoptic study of a case of alcoholic beri-beri is presented .
	manualset3
122582	3	404202	13	NULL	NULL	0	NULL	case	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A detailed clinical and autoptic study of a case of alcoholic beri-beri is presented .
	manualset3
122583	4	404202	13	NULL	NULL	0	NULL	alcoholic beri-beri 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A detailed clinical and autoptic study of a case of alcoholic beri-beri is presented .
	manualset3
122584	1	404203	13	NULL	NULL	0	NULL	One-year 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	One-year observation of kidney allograft recipients converted from cyclosporine microemulsion to tacrolimus .
	manualset3
122585	2	404203	13	NULL	NULL	0	NULL	observation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	One-year observation of kidney allograft recipients converted from cyclosporine microemulsion to tacrolimus .
	manualset3
122586	3	404203	13	NULL	NULL	0	NULL	kidney allograft recipients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One-year observation of kidney allograft recipients converted from cyclosporine microemulsion to tacrolimus .
	manualset3
122587	4	404203	13	NULL	NULL	0	NULL	cyclosporine microemulsion	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	One-year observation of kidney allograft recipients converted from cyclosporine microemulsion to tacrolimus .
	manualset3
122588	5	404203	13	NULL	NULL	0	NULL	tacrolimus	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	One-year observation of kidney allograft recipients converted from cyclosporine microemulsion to tacrolimus .
	manualset3
122589	1	404204	13	NULL	NULL	0	NULL	One ( Group I ) 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One ( Group I ) was composed of 21 patients who were given the antimalarial drug as part of the first-line therapy , either with a corticosteroid in a mean dose of 36 mg/d ( 18 patients ) or with a nonsteroidal antiinflammatory agent .
	manualset3
122590	2	404204	13	NULL	NULL	0	NULL	21 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One ( Group I ) was composed of 21 patients who were given the antimalarial drug as part of the first-line therapy , either with a corticosteroid in a mean dose of 36 mg/d ( 18 patients ) or with a nonsteroidal antiinflammatory agent .
	manualset3
122591	3	404204	13	NULL	NULL	0	NULL	antimalarial drug 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	One ( Group I ) was composed of 21 patients who were given the antimalarial drug as part of the first-line therapy , either with a corticosteroid in a mean dose of 36 mg/d ( 18 patients ) or with a nonsteroidal antiinflammatory agent .
	manualset3
122592	4	404204	13	NULL	NULL	0	NULL	first-line therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	One ( Group I ) was composed of 21 patients who were given the antimalarial drug as part of the first-line therapy , either with a corticosteroid in a mean dose of 36 mg/d ( 18 patients ) or with a nonsteroidal antiinflammatory agent .
	manualset3
122593	5	404204	13	NULL	NULL	0	NULL	corticosteroid	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	One ( Group I ) was composed of 21 patients who were given the antimalarial drug as part of the first-line therapy , either with a corticosteroid in a mean dose of 36 mg/d ( 18 patients ) or with a nonsteroidal antiinflammatory agent .
	manualset3
122594	6	404204	13	NULL	NULL	0	NULL	mean dose	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One ( Group I ) was composed of 21 patients who were given the antimalarial drug as part of the first-line therapy , either with a corticosteroid in a mean dose of 36 mg/d ( 18 patients ) or with a nonsteroidal antiinflammatory agent .
	manualset3
122595	7	404204	13	NULL	NULL	0	NULL	36 mg/d	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One ( Group I ) was composed of 21 patients who were given the antimalarial drug as part of the first-line therapy , either with a corticosteroid in a mean dose of 36 mg/d ( 18 patients ) or with a nonsteroidal antiinflammatory agent .
	manualset3
122596	8	404204	13	NULL	NULL	0	NULL	18 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One ( Group I ) was composed of 21 patients who were given the antimalarial drug as part of the first-line therapy , either with a corticosteroid in a mean dose of 36 mg/d ( 18 patients ) or with a nonsteroidal antiinflammatory agent .
	manualset3
122597	9	404204	13	NULL	NULL	0	NULL	nonsteroidal antiinflammatory agent	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	One ( Group I ) was composed of 21 patients who were given the antimalarial drug as part of the first-line therapy , either with a corticosteroid in a mean dose of 36 mg/d ( 18 patients ) or with a nonsteroidal antiinflammatory agent .
	manualset3
122598	1	404205	13	NULL	NULL	0	NULL	One -dimensional SDS-PAGE zymography 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	One - and two-dimensional SDS-PAGE zymography with quenched fluorogenic substrates provides identification of biological fluid proteases by direct mass spectrometry .
	manualset3
122599	2	404205	13	NULL	NULL	0	NULL	two-dimensional SDS-PAGE zymography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	One - and two-dimensional SDS-PAGE zymography with quenched fluorogenic substrates provides identification of biological fluid proteases by direct mass spectrometry .
	manualset3
122600	3	404205	13	NULL	NULL	0	NULL	fluorogenic substrates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	One - and two-dimensional SDS-PAGE zymography with quenched fluorogenic substrates provides identification of biological fluid proteases by direct mass spectrometry .
	manualset3
122601	4	404205	13	NULL	NULL	0	NULL	identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One - and two-dimensional SDS-PAGE zymography with quenched fluorogenic substrates provides identification of biological fluid proteases by direct mass spectrometry .
	manualset3
122602	5	404205	13	NULL	NULL	0	NULL	 biological fluid proteases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One - and two-dimensional SDS-PAGE zymography with quenched fluorogenic substrates provides identification of biological fluid proteases by direct mass spectrometry .
	manualset3
122603	6	404205	13	NULL	NULL	0	NULL	direct mass spectrometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	One - and two-dimensional SDS-PAGE zymography with quenched fluorogenic substrates provides identification of biological fluid proteases by direct mass spectrometry .
	manualset3
122604	1	404206	13	NULL	NULL	0	NULL	ETC protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One ETC protein was present at higher levels in broilers without PHS than in broilers with PHS in both lines , and one ETC protein was present at lower levels in susceptible line birds without PHS than in susceptible line birds with PHS or in resistant line birds with or without PHS .
	manualset3
122605	2	404206	13	NULL	NULL	0	NULL	levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One ETC protein was present at higher levels in broilers without PHS than in broilers with PHS in both lines , and one ETC protein was present at lower levels in susceptible line birds without PHS than in susceptible line birds with PHS or in resistant line birds with or without PHS .
	manualset3
122606	3	404206	13	NULL	NULL	0	NULL	broilers	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	One ETC protein was present at higher levels in broilers without PHS than in broilers with PHS in both lines , and one ETC protein was present at lower levels in susceptible line birds without PHS than in susceptible line birds with PHS or in resistant line birds with or without PHS .
	manualset3
122607	4	404206	13	NULL	NULL	0	NULL	PHS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	One ETC protein was present at higher levels in broilers without PHS than in broilers with PHS in both lines , and one ETC protein was present at lower levels in susceptible line birds without PHS than in susceptible line birds with PHS or in resistant line birds with or without PHS .
	manualset3
122608	5	404206	13	NULL	NULL	0	NULL	broilers	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	One ETC protein was present at higher levels in broilers without PHS than in broilers with PHS in both lines , and one ETC protein was present at lower levels in susceptible line birds without PHS than in susceptible line birds with PHS or in resistant line birds with or without PHS .
	manualset3
122609	6	404206	13	NULL	NULL	0	NULL	PHS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	One ETC protein was present at higher levels in broilers without PHS than in broilers with PHS in both lines , and one ETC protein was present at lower levels in susceptible line birds without PHS than in susceptible line birds with PHS or in resistant line birds with or without PHS .
	manualset3
122610	7	404206	13	NULL	NULL	0	NULL	lines	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	One ETC protein was present at higher levels in broilers without PHS than in broilers with PHS in both lines , and one ETC protein was present at lower levels in susceptible line birds without PHS than in susceptible line birds with PHS or in resistant line birds with or without PHS .
	manualset3
122611	8	404206	13	NULL	NULL	0	NULL	ETC protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One ETC protein was present at higher levels in broilers without PHS than in broilers with PHS in both lines , and one ETC protein was present at lower levels in susceptible line birds without PHS than in susceptible line birds with PHS or in resistant line birds with or without PHS .
	manualset3
122612	9	404206	13	NULL	NULL	0	NULL	levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One ETC protein was present at higher levels in broilers without PHS than in broilers with PHS in both lines , and one ETC protein was present at lower levels in susceptible line birds without PHS than in susceptible line birds with PHS or in resistant line birds with or without PHS .
	manualset3
122613	10	404206	13	NULL	NULL	0	NULL	susceptible line birds	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	One ETC protein was present at higher levels in broilers without PHS than in broilers with PHS in both lines , and one ETC protein was present at lower levels in susceptible line birds without PHS than in susceptible line birds with PHS or in resistant line birds with or without PHS .
	manualset3
122614	11	404206	13	NULL	NULL	0	NULL	PHS 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	One ETC protein was present at higher levels in broilers without PHS than in broilers with PHS in both lines , and one ETC protein was present at lower levels in susceptible line birds without PHS than in susceptible line birds with PHS or in resistant line birds with or without PHS .
	manualset3
122615	12	404206	13	NULL	NULL	0	NULL	susceptible line birds	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	One ETC protein was present at higher levels in broilers without PHS than in broilers with PHS in both lines , and one ETC protein was present at lower levels in susceptible line birds without PHS than in susceptible line birds with PHS or in resistant line birds with or without PHS .
	manualset3
122616	13	404206	13	NULL	NULL	0	NULL	PHS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	One ETC protein was present at higher levels in broilers without PHS than in broilers with PHS in both lines , and one ETC protein was present at lower levels in susceptible line birds without PHS than in susceptible line birds with PHS or in resistant line birds with or without PHS .
	manualset3
122617	14	404206	13	NULL	NULL	0	NULL	resistant line birds 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	One ETC protein was present at higher levels in broilers without PHS than in broilers with PHS in both lines , and one ETC protein was present at lower levels in susceptible line birds without PHS than in susceptible line birds with PHS or in resistant line birds with or without PHS .
	manualset3
122618	15	404206	13	NULL	NULL	0	NULL	PHS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	One ETC protein was present at higher levels in broilers without PHS than in broilers with PHS in both lines , and one ETC protein was present at lower levels in susceptible line birds without PHS than in susceptible line birds with PHS or in resistant line birds with or without PHS .
	manualset3
123042	16	404206	13	NULL	NULL	0	NULL	One 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One ETC protein was present at higher levels in broilers without PHS than in broilers with PHS in both lines , and one ETC protein was present at lower levels in susceptible line birds without PHS than in susceptible line birds with PHS or in resistant line birds with or without PHS .
	manualset3
122619	1	404207	13	NULL	NULL	0	NULL	IPSF 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One IPSF named IPSF-II alpha was purified and identified as glyceraldehyde-3-phosphate dehydrogenase as previously reported .
	manualset3
122620	2	404207	13	NULL	NULL	0	NULL	IPSF-II alpha 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One IPSF named IPSF-II alpha was purified and identified as glyceraldehyde-3-phosphate dehydrogenase as previously reported .
	manualset3
122621	3	404207	13	NULL	NULL	0	NULL	glyceraldehyde-3-phosphate dehydrogenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One IPSF named IPSF-II alpha was purified and identified as glyceraldehyde-3-phosphate dehydrogenase as previously reported .
	manualset3
123041	4	404207	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One IPSF named IPSF-II alpha was purified and identified as glyceraldehyde-3-phosphate dehydrogenase as previously reported .
	manualset3
122622	1	404208	13	NULL	NULL	0	NULL	aim	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One aim of the present study was to demonstrate in the laboratory that TO reduces stuttering in children .
	manualset3
122623	2	404208	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	One aim of the present study was to demonstrate in the laboratory that TO reduces stuttering in children .
	manualset3
122624	3	404208	13	NULL	NULL	0	NULL	laboratory	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	One aim of the present study was to demonstrate in the laboratory that TO reduces stuttering in children .
	manualset3
122625	4	404208	13	NULL	NULL	0	NULL	TO	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One aim of the present study was to demonstrate in the laboratory that TO reduces stuttering in children .
	manualset3
122626	5	404208	13	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One aim of the present study was to demonstrate in the laboratory that TO reduces stuttering in children .
	manualset3
122627	1	404209	13	NULL	NULL	0	NULL	aneurysm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One aneurysm out of 25 treated with the combination of a stent and Onyx showed recanalization .
	manualset3
122628	2	404209	13	NULL	NULL	0	NULL	25	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One aneurysm out of 25 treated with the combination of a stent and Onyx showed recanalization .
	manualset3
122629	3	404209	13	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One aneurysm out of 25 treated with the combination of a stent and Onyx showed recanalization .
	manualset3
122630	4	404209	13	NULL	NULL	0	NULL	stent	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	One aneurysm out of 25 treated with the combination of a stent and Onyx showed recanalization .
	manualset3
122631	5	404209	13	NULL	NULL	0	NULL	Onyx	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	One aneurysm out of 25 treated with the combination of a stent and Onyx showed recanalization .
	manualset3
122632	6	404209	13	NULL	NULL	0	NULL	recanalization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One aneurysm out of 25 treated with the combination of a stent and Onyx showed recanalization .
	manualset3
123040	7	404209	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One aneurysm out of 25 treated with the combination of a stent and Onyx showed recanalization .
	manualset3
122633	1	404210	13	NULL	NULL	0	NULL	Blood vessels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Blood vessels of the myocardial microcirculatory bed after radical correction of tetralogy of Fallot ) .
	manualset3
122634	2	404210	13	NULL	NULL	0	NULL	myocardial microcirculatory bed	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Blood vessels of the myocardial microcirculatory bed after radical correction of tetralogy of Fallot ) .
	manualset3
122635	3	404210	13	NULL	NULL	0	NULL	radical correction 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Blood vessels of the myocardial microcirculatory bed after radical correction of tetralogy of Fallot ) .
	manualset3
122636	4	404210	13	NULL	NULL	0	NULL	tetralogy of Fallot	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Blood vessels of the myocardial microcirculatory bed after radical correction of tetralogy of Fallot ) .
	manualset3
122637	1	404211	13	NULL	NULL	0	NULL	antigen	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	One antigen is defined by a monoclonal antibody which is subsequently detected by binding bovine red blood cells coated with a suitable antibody .
	manualset3
122638	2	404211	13	NULL	NULL	0	NULL	monoclonal antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One antigen is defined by a monoclonal antibody which is subsequently detected by binding bovine red blood cells coated with a suitable antibody .
	manualset3
122639	3	404211	13	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One antigen is defined by a monoclonal antibody which is subsequently detected by binding bovine red blood cells coated with a suitable antibody .
	manualset3
122640	4	404211	13	NULL	NULL	0	NULL	bovine red blood cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	One antigen is defined by a monoclonal antibody which is subsequently detected by binding bovine red blood cells coated with a suitable antibody .
	manualset3
122641	5	404211	13	NULL	NULL	0	NULL	antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One antigen is defined by a monoclonal antibody which is subsequently detected by binding bovine red blood cells coated with a suitable antibody .
	manualset3
123039	6	404211	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One antigen is defined by a monoclonal antibody which is subsequently detected by binding bovine red blood cells coated with a suitable antibody .
	manualset3
122642	1	404212	13	NULL	NULL	0	NULL	approach 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One approach to assess the relevance of his ideas to medical science has been to evaluate examples of successful research .
	manualset3
122643	2	404212	13	NULL	NULL	0	NULL	relevance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One approach to assess the relevance of his ideas to medical science has been to evaluate examples of successful research .
	manualset3
122644	3	404212	13	NULL	NULL	0	NULL	ideas	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One approach to assess the relevance of his ideas to medical science has been to evaluate examples of successful research .
	manualset3
122645	4	404212	13	NULL	NULL	0	NULL	medical science	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	One approach to assess the relevance of his ideas to medical science has been to evaluate examples of successful research .
	manualset3
122646	5	404212	13	NULL	NULL	0	NULL	examples	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One approach to assess the relevance of his ideas to medical science has been to evaluate examples of successful research .
	manualset3
122647	6	404212	13	NULL	NULL	0	NULL	successful research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	One approach to assess the relevance of his ideas to medical science has been to evaluate examples of successful research .
	manualset3
123038	7	404212	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One approach to assess the relevance of his ideas to medical science has been to evaluate examples of successful research .
	manualset3
122648	1	404213	13	NULL	NULL	0	NULL	breakpoint diameter	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One can thus estimate the breakpoint diameter for a given MIC breakpoint ; for example , an MIC breakpoint of less than or equal to 4 micrograms/ml would correspond to a greater than or equal to 15-mm breakpoint diameter for vancomycin ( 30-microgram disk ) and a greater than or equal to 13-mm breakpoint diameter for teicoplanin ( 30-microgram disk ) .
	manualset3
122649	2	404213	13	NULL	NULL	0	NULL	MIC breakpoint	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One can thus estimate the breakpoint diameter for a given MIC breakpoint ; for example , an MIC breakpoint of less than or equal to 4 micrograms/ml would correspond to a greater than or equal to 15-mm breakpoint diameter for vancomycin ( 30-microgram disk ) and a greater than or equal to 13-mm breakpoint diameter for teicoplanin ( 30-microgram disk ) .
	manualset3
122650	3	404213	13	NULL	NULL	0	NULL	example	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One can thus estimate the breakpoint diameter for a given MIC breakpoint ; for example , an MIC breakpoint of less than or equal to 4 micrograms/ml would correspond to a greater than or equal to 15-mm breakpoint diameter for vancomycin ( 30-microgram disk ) and a greater than or equal to 13-mm breakpoint diameter for teicoplanin ( 30-microgram disk ) .
	manualset3
122651	4	404213	13	NULL	NULL	0	NULL	MIC breakpoint	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One can thus estimate the breakpoint diameter for a given MIC breakpoint ; for example , an MIC breakpoint of less than or equal to 4 micrograms/ml would correspond to a greater than or equal to 15-mm breakpoint diameter for vancomycin ( 30-microgram disk ) and a greater than or equal to 13-mm breakpoint diameter for teicoplanin ( 30-microgram disk ) .
	manualset3
122652	5	404213	13	NULL	NULL	0	NULL	less than or equal to 4 micrograms/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One can thus estimate the breakpoint diameter for a given MIC breakpoint ; for example , an MIC breakpoint of less than or equal to 4 micrograms/ml would correspond to a greater than or equal to 15-mm breakpoint diameter for vancomycin ( 30-microgram disk ) and a greater than or equal to 13-mm breakpoint diameter for teicoplanin ( 30-microgram disk ) .
	manualset3
122653	6	404213	13	NULL	NULL	NULL	NULL	greater than or equal to 15-mm	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	One can thus estimate the breakpoint diameter for a given MIC breakpoint ; for example , an MIC breakpoint of less than or equal to 4 micrograms/ml would correspond to a greater than or equal to 15-mm breakpoint diameter for vancomycin ( 30-microgram disk ) and a greater than or equal to 13-mm breakpoint diameter for teicoplanin ( 30-microgram disk ) .
	manualset3
122654	7	404213	13	NULL	NULL	0	NULL	breakpoint diameter	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One can thus estimate the breakpoint diameter for a given MIC breakpoint ; for example , an MIC breakpoint of less than or equal to 4 micrograms/ml would correspond to a greater than or equal to 15-mm breakpoint diameter for vancomycin ( 30-microgram disk ) and a greater than or equal to 13-mm breakpoint diameter for teicoplanin ( 30-microgram disk ) .
	manualset3
122655	8	404213	13	NULL	NULL	0	NULL	vancomycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	One can thus estimate the breakpoint diameter for a given MIC breakpoint ; for example , an MIC breakpoint of less than or equal to 4 micrograms/ml would correspond to a greater than or equal to 15-mm breakpoint diameter for vancomycin ( 30-microgram disk ) and a greater than or equal to 13-mm breakpoint diameter for teicoplanin ( 30-microgram disk ) .
	manualset3
122656	9	404213	13	NULL	NULL	0	NULL	30-microgram disk 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One can thus estimate the breakpoint diameter for a given MIC breakpoint ; for example , an MIC breakpoint of less than or equal to 4 micrograms/ml would correspond to a greater than or equal to 15-mm breakpoint diameter for vancomycin ( 30-microgram disk ) and a greater than or equal to 13-mm breakpoint diameter for teicoplanin ( 30-microgram disk ) .
	manualset3
122657	10	404213	13	NULL	NULL	NULL	NULL	greater than or equal to 13-mm	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	One can thus estimate the breakpoint diameter for a given MIC breakpoint ; for example , an MIC breakpoint of less than or equal to 4 micrograms/ml would correspond to a greater than or equal to 15-mm breakpoint diameter for vancomycin ( 30-microgram disk ) and a greater than or equal to 13-mm breakpoint diameter for teicoplanin ( 30-microgram disk ) .
	manualset3
122658	11	404213	13	NULL	NULL	0	NULL	breakpoint diameter 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One can thus estimate the breakpoint diameter for a given MIC breakpoint ; for example , an MIC breakpoint of less than or equal to 4 micrograms/ml would correspond to a greater than or equal to 15-mm breakpoint diameter for vancomycin ( 30-microgram disk ) and a greater than or equal to 13-mm breakpoint diameter for teicoplanin ( 30-microgram disk ) .
	manualset3
122659	12	404213	13	NULL	NULL	0	NULL	teicoplanin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	One can thus estimate the breakpoint diameter for a given MIC breakpoint ; for example , an MIC breakpoint of less than or equal to 4 micrograms/ml would correspond to a greater than or equal to 15-mm breakpoint diameter for vancomycin ( 30-microgram disk ) and a greater than or equal to 13-mm breakpoint diameter for teicoplanin ( 30-microgram disk ) .
	manualset3
122660	13	404213	13	NULL	NULL	0	NULL	30-microgram disk	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One can thus estimate the breakpoint diameter for a given MIC breakpoint ; for example , an MIC breakpoint of less than or equal to 4 micrograms/ml would correspond to a greater than or equal to 15-mm breakpoint diameter for vancomycin ( 30-microgram disk ) and a greater than or equal to 13-mm breakpoint diameter for teicoplanin ( 30-microgram disk ) .
	manualset3
122661	1	404214	13	NULL	NULL	0	NULL	carrier	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	One carrier found compound heterozygous for TTR D99N and L111M ( Leu111Met ) associated with cardiac amyloid is asymptomatic ( 42 years ) .
	manualset3
122662	2	404214	13	NULL	NULL	NULL	NULL	compound	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	One carrier found compound heterozygous for TTR D99N and L111M ( Leu111Met ) associated with cardiac amyloid is asymptomatic ( 42 years ) .
	manualset3
122663	3	404214	13	NULL	NULL	NULL	NULL	TTR D99N 	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	One carrier found compound heterozygous for TTR D99N and L111M ( Leu111Met ) associated with cardiac amyloid is asymptomatic ( 42 years ) .
	manualset3
122664	4	404214	13	NULL	NULL	NULL	NULL	TTR L111M ( Leu111Met )	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	One carrier found compound heterozygous for TTR D99N and L111M ( Leu111Met ) associated with cardiac amyloid is asymptomatic ( 42 years ) .
	manualset3
122665	5	404214	13	NULL	NULL	0	NULL	cardiac amyloid	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One carrier found compound heterozygous for TTR D99N and L111M ( Leu111Met ) associated with cardiac amyloid is asymptomatic ( 42 years ) .
	manualset3
122666	6	404214	13	NULL	NULL	0	NULL	42 years	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One carrier found compound heterozygous for TTR D99N and L111M ( Leu111Met ) associated with cardiac amyloid is asymptomatic ( 42 years ) .
	manualset3
123037	7	404214	13	NULL	NULL	0	NULL	One 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One carrier found compound heterozygous for TTR D99N and L111M ( Leu111Met ) associated with cardiac amyloid is asymptomatic ( 42 years ) .
	manualset3
122667	1	404215	13	NULL	NULL	0	NULL	child	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	One child has received a cochlear implant , and another will be implanted shortly .
	manualset3
122668	2	404215	13	NULL	NULL	0	NULL	cochlear implant	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	One child has received a cochlear implant , and another will be implanted shortly .
	manualset3
123036	3	404215	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One child has received a cochlear implant , and another will be implanted shortly .
	manualset3
122669	1	404216	13	NULL	NULL	0	NULL	child	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	One child required reoperation because of graft thrombosis and an aortic homograft was used in him on the second occasion .
	manualset3
122670	2	404216	13	NULL	NULL	0	NULL	reoperation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	One child required reoperation because of graft thrombosis and an aortic homograft was used in him on the second occasion .
	manualset3
122671	3	404216	13	NULL	NULL	0	NULL	graft thrombosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One child required reoperation because of graft thrombosis and an aortic homograft was used in him on the second occasion .
	manualset3
122672	4	404216	13	NULL	NULL	0	NULL	aortic homograft	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	One child required reoperation because of graft thrombosis and an aortic homograft was used in him on the second occasion .
	manualset3
122673	5	404216	13	NULL	NULL	0	NULL	second occasion	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	One child required reoperation because of graft thrombosis and an aortic homograft was used in him on the second occasion .
	manualset3
123035	6	404216	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One child required reoperation because of graft thrombosis and an aortic homograft was used in him on the second occasion .
	manualset3
122674	1	404217	13	NULL	NULL	0	NULL	corollary	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One corollary of this idea is that CTL should recognize appropriate short peptides on the target cell surface .
	manualset3
122675	2	404217	13	NULL	NULL	0	NULL	idea	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One corollary of this idea is that CTL should recognize appropriate short peptides on the target cell surface .
	manualset3
122676	3	404217	13	NULL	NULL	0	NULL	CTL 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	One corollary of this idea is that CTL should recognize appropriate short peptides on the target cell surface .
	manualset3
122677	4	404217	13	NULL	NULL	0	NULL	short peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	One corollary of this idea is that CTL should recognize appropriate short peptides on the target cell surface .
	manualset3
122678	5	404217	13	NULL	NULL	0	NULL	target cell surface	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	One corollary of this idea is that CTL should recognize appropriate short peptides on the target cell surface .
	manualset3
122679	1	404218	13	NULL	NULL	0	NULL	structural analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A detailed structural analysis of mutant spores has been performed to gain insight into the specific aspects of spore differentiation in which SrfA is involved .
	manualset3
122680	2	404218	13	NULL	NULL	0	NULL	mutant spores 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A detailed structural analysis of mutant spores has been performed to gain insight into the specific aspects of spore differentiation in which SrfA is involved .
	manualset3
122681	3	404218	13	NULL	NULL	0	NULL	insight	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A detailed structural analysis of mutant spores has been performed to gain insight into the specific aspects of spore differentiation in which SrfA is involved .
	manualset3
122682	4	404218	13	NULL	NULL	0	NULL	aspects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A detailed structural analysis of mutant spores has been performed to gain insight into the specific aspects of spore differentiation in which SrfA is involved .
	manualset3
122683	5	404218	13	NULL	NULL	0	NULL	spore differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A detailed structural analysis of mutant spores has been performed to gain insight into the specific aspects of spore differentiation in which SrfA is involved .
	manualset3
122684	6	404218	13	NULL	NULL	0	NULL	SrfA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A detailed structural analysis of mutant spores has been performed to gain insight into the specific aspects of spore differentiation in which SrfA is involved .
	manualset3
122685	1	404219	13	NULL	NULL	0	NULL	dimension	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One dimension was found that was related positively to the husbands ' needs for Dominance , Affiliation , Heterosexuality , Exhibition , and Change , whereas the same dimension was related positively to the wives ' needs for Achievement , Dominance , Endurance , and Intraception .
	manualset3
122686	2	404219	13	NULL	NULL	0	NULL	husbands '	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One dimension was found that was related positively to the husbands ' needs for Dominance , Affiliation , Heterosexuality , Exhibition , and Change , whereas the same dimension was related positively to the wives ' needs for Achievement , Dominance , Endurance , and Intraception .
	manualset3
122687	3	404219	13	NULL	NULL	NULL	NULL	Dominance	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	One dimension was found that was related positively to the husbands ' needs for Dominance , Affiliation , Heterosexuality , Exhibition , and Change , whereas the same dimension was related positively to the wives ' needs for Achievement , Dominance , Endurance , and Intraception .
	manualset3
122688	4	404219	13	NULL	NULL	0	NULL	needs 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One dimension was found that was related positively to the husbands ' needs for Dominance , Affiliation , Heterosexuality , Exhibition , and Change , whereas the same dimension was related positively to the wives ' needs for Achievement , Dominance , Endurance , and Intraception .
	manualset3
122689	5	404219	13	NULL	NULL	0	NULL	Affiliation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One dimension was found that was related positively to the husbands ' needs for Dominance , Affiliation , Heterosexuality , Exhibition , and Change , whereas the same dimension was related positively to the wives ' needs for Achievement , Dominance , Endurance , and Intraception .
	manualset3
122690	6	404219	13	NULL	NULL	0	NULL	Heterosexuality	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One dimension was found that was related positively to the husbands ' needs for Dominance , Affiliation , Heterosexuality , Exhibition , and Change , whereas the same dimension was related positively to the wives ' needs for Achievement , Dominance , Endurance , and Intraception .
	manualset3
122691	7	404219	13	NULL	NULL	0	NULL	Exhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One dimension was found that was related positively to the husbands ' needs for Dominance , Affiliation , Heterosexuality , Exhibition , and Change , whereas the same dimension was related positively to the wives ' needs for Achievement , Dominance , Endurance , and Intraception .
	manualset3
122692	8	404219	13	NULL	NULL	0	NULL	Change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One dimension was found that was related positively to the husbands ' needs for Dominance , Affiliation , Heterosexuality , Exhibition , and Change , whereas the same dimension was related positively to the wives ' needs for Achievement , Dominance , Endurance , and Intraception .
	manualset3
122693	9	404219	13	NULL	NULL	0	NULL	dimension 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One dimension was found that was related positively to the husbands ' needs for Dominance , Affiliation , Heterosexuality , Exhibition , and Change , whereas the same dimension was related positively to the wives ' needs for Achievement , Dominance , Endurance , and Intraception .
	manualset3
122694	10	404219	13	NULL	NULL	0	NULL	wives '	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One dimension was found that was related positively to the husbands ' needs for Dominance , Affiliation , Heterosexuality , Exhibition , and Change , whereas the same dimension was related positively to the wives ' needs for Achievement , Dominance , Endurance , and Intraception .
	manualset3
122695	11	404219	13	NULL	NULL	0	NULL	Achievement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One dimension was found that was related positively to the husbands ' needs for Dominance , Affiliation , Heterosexuality , Exhibition , and Change , whereas the same dimension was related positively to the wives ' needs for Achievement , Dominance , Endurance , and Intraception .
	manualset3
122696	12	404219	13	NULL	NULL	0	NULL	Dominance 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One dimension was found that was related positively to the husbands ' needs for Dominance , Affiliation , Heterosexuality , Exhibition , and Change , whereas the same dimension was related positively to the wives ' needs for Achievement , Dominance , Endurance , and Intraception .
	manualset3
122698	14	404219	13	NULL	NULL	0	NULL	Intraception 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One dimension was found that was related positively to the husbands ' needs for Dominance , Affiliation , Heterosexuality , Exhibition , and Change , whereas the same dimension was related positively to the wives ' needs for Achievement , Dominance , Endurance , and Intraception .
	manualset3
123034	15	404219	13	NULL	NULL	0	NULL	One 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One dimension was found that was related positively to the husbands ' needs for Dominance , Affiliation , Heterosexuality , Exhibition , and Change , whereas the same dimension was related positively to the wives ' needs for Achievement , Dominance , Endurance , and Intraception .
	manualset3
122697	1	404220	13	NULL	NULL	NULL	NULL	feature of glioblastoma	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	One feature of glioblastoma associated with poor prognosis is the degree of hypoxia and expression levels of hypoxia-inducible factor-1 ( HIF-1 ) .
	manualset3
122699	2	404220	13	NULL	NULL	0	NULL	prognosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One feature of glioblastoma associated with poor prognosis is the degree of hypoxia and expression levels of hypoxia-inducible factor-1 ( HIF-1 ) .
	manualset3
122700	3	404220	13	NULL	NULL	0	NULL	degree of hypoxia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One feature of glioblastoma associated with poor prognosis is the degree of hypoxia and expression levels of hypoxia-inducible factor-1 ( HIF-1 ) .
	manualset3
122701	4	404220	13	NULL	NULL	0	NULL	expression levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One feature of glioblastoma associated with poor prognosis is the degree of hypoxia and expression levels of hypoxia-inducible factor-1 ( HIF-1 ) .
	manualset3
122702	5	404220	13	NULL	NULL	0	NULL	hypoxia-inducible factor-1 ( HIF-1 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One feature of glioblastoma associated with poor prognosis is the degree of hypoxia and expression levels of hypoxia-inducible factor-1 ( HIF-1 ) .
	manualset3
123033	6	404220	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One feature of glioblastoma associated with poor prognosis is the degree of hypoxia and expression levels of hypoxia-inducible factor-1 ( HIF-1 ) .
	manualset3
122801	1	404221	13	NULL	NULL	0	NULL	fetus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	One fetus showed an intermediate form of cardiac malformation with a hypoplastic cor triloculare .
	manualset3
122802	2	404221	13	NULL	NULL	0	NULL	intermediate form of cardiac malformation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One fetus showed an intermediate form of cardiac malformation with a hypoplastic cor triloculare .
	manualset3
122803	3	404221	13	NULL	NULL	0	NULL	hypoplastic cor triloculare	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One fetus showed an intermediate form of cardiac malformation with a hypoplastic cor triloculare .
	manualset3
123032	4	404221	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One fetus showed an intermediate form of cardiac malformation with a hypoplastic cor triloculare .
	manualset3
122804	1	404222	13	NULL	NULL	0	NULL	gestational sac	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	One gestational sac , together with regular heart activity , was recorded by ultrasonography at 8 weeks of gestation .
	manualset3
122805	2	404222	13	NULL	NULL	0	NULL	regular heart activity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One gestational sac , together with regular heart activity , was recorded by ultrasonography at 8 weeks of gestation .
	manualset3
122806	3	404222	13	NULL	NULL	0	NULL	ultrasonography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	One gestational sac , together with regular heart activity , was recorded by ultrasonography at 8 weeks of gestation .
	manualset3
122807	4	404222	13	NULL	NULL	0	NULL	8 weeks of gestation 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	One gestational sac , together with regular heart activity , was recorded by ultrasonography at 8 weeks of gestation .
	manualset3
123031	5	404222	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One gestational sac , together with regular heart activity , was recorded by ultrasonography at 8 weeks of gestation .
	manualset3
122817	1	404223	13	NULL	NULL	0	NULL	concern	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One great concern is the detection of Bacillus anthracis , the causative agent of anthrax .
	manualset3
122818	2	404223	13	NULL	NULL	0	NULL	detection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One great concern is the detection of Bacillus anthracis , the causative agent of anthrax .
	manualset3
122819	3	404223	13	NULL	NULL	0	NULL	Bacillus anthracis 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	One great concern is the detection of Bacillus anthracis , the causative agent of anthrax .
	manualset3
122820	4	404223	13	NULL	NULL	0	NULL	causative agent	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	One great concern is the detection of Bacillus anthracis , the causative agent of anthrax .
	manualset3
122821	5	404223	13	NULL	NULL	0	NULL	anthrax 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	One great concern is the detection of Bacillus anthracis , the causative agent of anthrax .
	manualset3
123030	6	404223	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One great concern is the detection of Bacillus anthracis , the causative agent of anthrax .
	manualset3
122822	1	404224	13	NULL	NULL	NULL	NULL	One group ( I )	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	One group ( I ) is genetically related to A. sobria ( type 208 ) .
	manualset3
122823	2	404224	13	NULL	NULL	0	NULL	A. sobria ( type 208 ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	One group ( I ) is genetically related to A. sobria ( type 208 ) .
	manualset3
122824	1	404225	13	NULL	NULL	0	NULL	One group 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	One group of male rats received LPS ( Salmonella minnesota ; 2 mg/kg , i.v. ) .
	manualset3
122825	2	404225	13	NULL	NULL	0	NULL	male rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	One group of male rats received LPS ( Salmonella minnesota ; 2 mg/kg , i.v. ) .
	manualset3
122826	3	404225	13	NULL	NULL	0	NULL	LPS	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	One group of male rats received LPS ( Salmonella minnesota ; 2 mg/kg , i.v. ) .
	manualset3
122828	4	404225	13	NULL	NULL	0	NULL	Salmonella minnesota	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	One group of male rats received LPS ( Salmonella minnesota ; 2 mg/kg , i.v. ) .
	manualset3
122830	5	404225	13	NULL	NULL	0	NULL	2 mg/kg	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	One group of male rats received LPS ( Salmonella minnesota ; 2 mg/kg , i.v. ) .
	manualset3
122835	1	404226	13	NULL	NULL	0	NULL	One group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One group of normal elderly adults and two groups of cognitively impaired elderly adults were compared on an implicit and an explicit memory task .
	manualset3
122836	2	404226	13	NULL	NULL	0	NULL	normal elderly adults 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One group of normal elderly adults and two groups of cognitively impaired elderly adults were compared on an implicit and an explicit memory task .
	manualset3
122837	3	404226	13	NULL	NULL	0	NULL	two groups 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One group of normal elderly adults and two groups of cognitively impaired elderly adults were compared on an implicit and an explicit memory task .
	manualset3
122839	4	404226	13	NULL	NULL	0	NULL	cognitively impaired elderly adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One group of normal elderly adults and two groups of cognitively impaired elderly adults were compared on an implicit and an explicit memory task .
	manualset3
122841	5	404226	13	NULL	NULL	0	NULL	memory task 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	One group of normal elderly adults and two groups of cognitively impaired elderly adults were compared on an implicit and an explicit memory task .
	manualset3
122843	1	404227	13	NULL	NULL	0	NULL	One hip	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	One hip required premature total hip replacement .
	manualset3
122844	2	404227	13	NULL	NULL	0	NULL	total hip replacement 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	One hip required premature total hip replacement .
	manualset3
122846	1	404228	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A detailed study of these diseases can provide insight into the biochemistry of NF-kappaB activation as well as the role of NF-kappaB in human health .
	manualset3
122847	2	404228	13	NULL	NULL	0	NULL	diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A detailed study of these diseases can provide insight into the biochemistry of NF-kappaB activation as well as the role of NF-kappaB in human health .
	manualset3
122848	3	404228	13	NULL	NULL	0	NULL	insight	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A detailed study of these diseases can provide insight into the biochemistry of NF-kappaB activation as well as the role of NF-kappaB in human health .
	manualset3
122849	4	404228	13	NULL	NULL	0	NULL	biochemistry	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A detailed study of these diseases can provide insight into the biochemistry of NF-kappaB activation as well as the role of NF-kappaB in human health .
	manualset3
122850	5	404228	13	NULL	NULL	0	NULL	NF-kappaB activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A detailed study of these diseases can provide insight into the biochemistry of NF-kappaB activation as well as the role of NF-kappaB in human health .
	manualset3
122851	6	404228	13	NULL	NULL	0	NULL	role 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A detailed study of these diseases can provide insight into the biochemistry of NF-kappaB activation as well as the role of NF-kappaB in human health .
	manualset3
122852	7	404228	13	NULL	NULL	0	NULL	NF-kappaB	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A detailed study of these diseases can provide insight into the biochemistry of NF-kappaB activation as well as the role of NF-kappaB in human health .
	manualset3
122853	8	404228	13	NULL	NULL	0	NULL	human health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A detailed study of these diseases can provide insight into the biochemistry of NF-kappaB activation as well as the role of NF-kappaB in human health .
	manualset3
122859	1	404229	13	NULL	NULL	NULL	NULL	One hundred and thirteen	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	One hundred and thirteen primary ( n = 56 ) and metastatic ( n = 57 ) lesions were immunohistochemically stained for APC , E-cadherin , and beta-catenin .
	manualset3
122861	3	404229	13	NULL	NULL	NULL	NULL	n = 56	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	One hundred and thirteen primary ( n = 56 ) and metastatic ( n = 57 ) lesions were immunohistochemically stained for APC , E-cadherin , and beta-catenin .
	manualset3
122865	4	404229	13	NULL	NULL	NULL	NULL	metastatic lesions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	One hundred and thirteen primary ( n = 56 ) and metastatic ( n = 57 ) lesions were immunohistochemically stained for APC , E-cadherin , and beta-catenin .
	manualset3
122866	2	404229	13	NULL	NULL	0	NULL	primary lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred and thirteen primary ( n = 56 ) and metastatic ( n = 57 ) lesions were immunohistochemically stained for APC , E-cadherin , and beta-catenin .
	manualset3
122870	5	404229	13	NULL	NULL	0	NULL	n = 57	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred and thirteen primary ( n = 56 ) and metastatic ( n = 57 ) lesions were immunohistochemically stained for APC , E-cadherin , and beta-catenin .
	manualset3
122872	6	404229	13	NULL	NULL	0	NULL	APC	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred and thirteen primary ( n = 56 ) and metastatic ( n = 57 ) lesions were immunohistochemically stained for APC , E-cadherin , and beta-catenin .
	manualset3
122873	7	404229	13	NULL	NULL	0	NULL	E-cadherin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred and thirteen primary ( n = 56 ) and metastatic ( n = 57 ) lesions were immunohistochemically stained for APC , E-cadherin , and beta-catenin .
	manualset3
122875	8	404229	13	NULL	NULL	0	NULL	beta-catenin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred and thirteen primary ( n = 56 ) and metastatic ( n = 57 ) lesions were immunohistochemically stained for APC , E-cadherin , and beta-catenin .
	manualset3
122876	1	404230	13	NULL	NULL	0	NULL	One hundred	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred consecutive patients operated on for sciatica pain using microsurgical techniques between April 1984 and February 1985 were evaluated retrospectively .
	manualset3
122878	2	404230	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred consecutive patients operated on for sciatica pain using microsurgical techniques between April 1984 and February 1985 were evaluated retrospectively .
	manualset3
122880	3	404230	13	NULL	NULL	0	NULL	sciatica pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred consecutive patients operated on for sciatica pain using microsurgical techniques between April 1984 and February 1985 were evaluated retrospectively .
	manualset3
122881	4	404230	13	NULL	NULL	0	NULL	microsurgical techniques	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred consecutive patients operated on for sciatica pain using microsurgical techniques between April 1984 and February 1985 were evaluated retrospectively .
	manualset3
122883	5	404230	13	NULL	NULL	0	NULL	April 1984 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred consecutive patients operated on for sciatica pain using microsurgical techniques between April 1984 and February 1985 were evaluated retrospectively .
	manualset3
122885	6	404230	13	NULL	NULL	0	NULL	February 1985	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred consecutive patients operated on for sciatica pain using microsurgical techniques between April 1984 and February 1985 were evaluated retrospectively .
	manualset3
122900	1	404231	13	NULL	NULL	0	NULL	One hundred	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred first-degree relatives of patients with schizophrenia ( AS ) and 88 first-degree relatives of affective psychotic ( APA ) patients completed the Eysenck Personality Questionnaire which measures extraversion , neuroticism , psychoticism .
	manualset3
122902	2	404231	13	NULL	NULL	0	NULL	first-degree relatives	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred first-degree relatives of patients with schizophrenia ( AS ) and 88 first-degree relatives of affective psychotic ( APA ) patients completed the Eysenck Personality Questionnaire which measures extraversion , neuroticism , psychoticism .
	manualset3
122903	3	404231	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred first-degree relatives of patients with schizophrenia ( AS ) and 88 first-degree relatives of affective psychotic ( APA ) patients completed the Eysenck Personality Questionnaire which measures extraversion , neuroticism , psychoticism .
	manualset3
122908	4	404231	13	NULL	NULL	0	NULL	schizophrenia ( AS ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred first-degree relatives of patients with schizophrenia ( AS ) and 88 first-degree relatives of affective psychotic ( APA ) patients completed the Eysenck Personality Questionnaire which measures extraversion , neuroticism , psychoticism .
	manualset3
122909	5	404231	13	NULL	NULL	0	NULL	88 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred first-degree relatives of patients with schizophrenia ( AS ) and 88 first-degree relatives of affective psychotic ( APA ) patients completed the Eysenck Personality Questionnaire which measures extraversion , neuroticism , psychoticism .
	manualset3
122910	6	404231	13	NULL	NULL	0	NULL	first-degree relatives	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred first-degree relatives of patients with schizophrenia ( AS ) and 88 first-degree relatives of affective psychotic ( APA ) patients completed the Eysenck Personality Questionnaire which measures extraversion , neuroticism , psychoticism .
	manualset3
122911	7	404231	13	NULL	NULL	0	NULL	affective psychotic ( APA ) patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred first-degree relatives of patients with schizophrenia ( AS ) and 88 first-degree relatives of affective psychotic ( APA ) patients completed the Eysenck Personality Questionnaire which measures extraversion , neuroticism , psychoticism .
	manualset3
122912	8	404231	13	NULL	NULL	0	NULL	Eysenck Personality Questionnaire	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred first-degree relatives of patients with schizophrenia ( AS ) and 88 first-degree relatives of affective psychotic ( APA ) patients completed the Eysenck Personality Questionnaire which measures extraversion , neuroticism , psychoticism .
	manualset3
122913	9	404231	13	NULL	NULL	0	NULL	extraversion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred first-degree relatives of patients with schizophrenia ( AS ) and 88 first-degree relatives of affective psychotic ( APA ) patients completed the Eysenck Personality Questionnaire which measures extraversion , neuroticism , psychoticism .
	manualset3
122914	10	404231	13	NULL	NULL	0	NULL	neuroticism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred first-degree relatives of patients with schizophrenia ( AS ) and 88 first-degree relatives of affective psychotic ( APA ) patients completed the Eysenck Personality Questionnaire which measures extraversion , neuroticism , psychoticism .
	manualset3
122915	11	404231	13	NULL	NULL	0	NULL	psychoticism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred first-degree relatives of patients with schizophrenia ( AS ) and 88 first-degree relatives of affective psychotic ( APA ) patients completed the Eysenck Personality Questionnaire which measures extraversion , neuroticism , psychoticism .
	manualset3
122916	1	404232	13	NULL	NULL	0	NULL	18 : 2 n6/18 : 3 n3 ratio	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A dietary 18 : 2 n6/18 : 3 n3 ratio of 165 versus 1.8 caused higher n6 and lower n3 22-carbon fatty acid levels , without changing total 22-carbon fatty acid levels , in phosphatidylethanolamine and phosphatidylcholine from several neural membrane fractions .
	manualset3
122917	2	404232	13	NULL	NULL	0	NULL	165 versus 1.8	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A dietary 18 : 2 n6/18 : 3 n3 ratio of 165 versus 1.8 caused higher n6 and lower n3 22-carbon fatty acid levels , without changing total 22-carbon fatty acid levels , in phosphatidylethanolamine and phosphatidylcholine from several neural membrane fractions .
	manualset3
122921	3	404232	13	NULL	NULL	0	NULL	higher n6 22-carbon fatty acid levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A dietary 18 : 2 n6/18 : 3 n3 ratio of 165 versus 1.8 caused higher n6 and lower n3 22-carbon fatty acid levels , without changing total 22-carbon fatty acid levels , in phosphatidylethanolamine and phosphatidylcholine from several neural membrane fractions .
	manualset3
122922	4	404232	13	NULL	NULL	0	NULL	lower n3 22-carbon fatty acid levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A dietary 18 : 2 n6/18 : 3 n3 ratio of 165 versus 1.8 caused higher n6 and lower n3 22-carbon fatty acid levels , without changing total 22-carbon fatty acid levels , in phosphatidylethanolamine and phosphatidylcholine from several neural membrane fractions .
	manualset3
122923	5	404232	13	NULL	NULL	0	NULL	total 22-carbon fatty acid levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A dietary 18 : 2 n6/18 : 3 n3 ratio of 165 versus 1.8 caused higher n6 and lower n3 22-carbon fatty acid levels , without changing total 22-carbon fatty acid levels , in phosphatidylethanolamine and phosphatidylcholine from several neural membrane fractions .
	manualset3
122924	6	404232	13	NULL	NULL	0	NULL	phosphatidylethanolamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A dietary 18 : 2 n6/18 : 3 n3 ratio of 165 versus 1.8 caused higher n6 and lower n3 22-carbon fatty acid levels , without changing total 22-carbon fatty acid levels , in phosphatidylethanolamine and phosphatidylcholine from several neural membrane fractions .
	manualset3
122926	7	404232	13	NULL	NULL	0	NULL	phosphatidylcholine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A dietary 18 : 2 n6/18 : 3 n3 ratio of 165 versus 1.8 caused higher n6 and lower n3 22-carbon fatty acid levels , without changing total 22-carbon fatty acid levels , in phosphatidylethanolamine and phosphatidylcholine from several neural membrane fractions .
	manualset3
122927	8	404232	13	NULL	NULL	0	NULL	neural membrane fractions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A dietary 18 : 2 n6/18 : 3 n3 ratio of 165 versus 1.8 caused higher n6 and lower n3 22-carbon fatty acid levels , without changing total 22-carbon fatty acid levels , in phosphatidylethanolamine and phosphatidylcholine from several neural membrane fractions .
	manualset3
122931	1	404233	13	NULL	NULL	0	NULL	One hundred twenty-four 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred twenty-four untreated patients with stage B2 carcinoma had a five-year survival rate of 77 % , confirming the relatively high survival of this group of patients who are treated with surgery alone .
	manualset3
122932	2	404233	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred twenty-four untreated patients with stage B2 carcinoma had a five-year survival rate of 77 % , confirming the relatively high survival of this group of patients who are treated with surgery alone .
	manualset3
122933	3	404233	13	NULL	NULL	0	NULL	stage B2 carcinoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred twenty-four untreated patients with stage B2 carcinoma had a five-year survival rate of 77 % , confirming the relatively high survival of this group of patients who are treated with surgery alone .
	manualset3
122934	4	404233	13	NULL	NULL	0	NULL	five-year 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred twenty-four untreated patients with stage B2 carcinoma had a five-year survival rate of 77 % , confirming the relatively high survival of this group of patients who are treated with surgery alone .
	manualset3
122935	5	404233	13	NULL	NULL	0	NULL	survival rate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred twenty-four untreated patients with stage B2 carcinoma had a five-year survival rate of 77 % , confirming the relatively high survival of this group of patients who are treated with surgery alone .
	manualset3
122936	6	404233	13	NULL	NULL	0	NULL	77 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred twenty-four untreated patients with stage B2 carcinoma had a five-year survival rate of 77 % , confirming the relatively high survival of this group of patients who are treated with surgery alone .
	manualset3
122937	7	404233	13	NULL	NULL	0	NULL	survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred twenty-four untreated patients with stage B2 carcinoma had a five-year survival rate of 77 % , confirming the relatively high survival of this group of patients who are treated with surgery alone .
	manualset3
122938	8	404233	13	NULL	NULL	0	NULL	group of patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred twenty-four untreated patients with stage B2 carcinoma had a five-year survival rate of 77 % , confirming the relatively high survival of this group of patients who are treated with surgery alone .
	manualset3
122939	9	404233	13	NULL	NULL	0	NULL	surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	One hundred twenty-four untreated patients with stage B2 carcinoma had a five-year survival rate of 77 % , confirming the relatively high survival of this group of patients who are treated with surgery alone .
	manualset3
122940	1	404234	13	NULL	NULL	0	NULL	intermolecular C-H ... O = C close contact	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One intermolecular C-H ... O = C close contact exists for the carboxyl group of one of the molecules .
	manualset3
122941	2	404234	13	NULL	NULL	0	NULL	carboxyl group	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	One intermolecular C-H ... O = C close contact exists for the carboxyl group of one of the molecules .
	manualset3
122942	3	404234	13	NULL	NULL	0	NULL	molecules 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	One intermolecular C-H ... O = C close contact exists for the carboxyl group of one of the molecules .
	manualset3
123029	4	404234	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One intermolecular C-H ... O = C close contact exists for the carboxyl group of one of the molecules .
	manualset3
122943	1	404235	13	NULL	NULL	0	NULL	issue	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One issue that has received little consideration so far is whether the hippocampus can function normally in the presence of a lesion to perirhinal cortex that produces noticeable memory impairments .
	manualset3
122944	2	404235	13	NULL	NULL	0	NULL	consideration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One issue that has received little consideration so far is whether the hippocampus can function normally in the presence of a lesion to perirhinal cortex that produces noticeable memory impairments .
	manualset3
122945	3	404235	13	NULL	NULL	0	NULL	hippocampus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	One issue that has received little consideration so far is whether the hippocampus can function normally in the presence of a lesion to perirhinal cortex that produces noticeable memory impairments .
	manualset3
122946	4	404235	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One issue that has received little consideration so far is whether the hippocampus can function normally in the presence of a lesion to perirhinal cortex that produces noticeable memory impairments .
	manualset3
122947	5	404235	13	NULL	NULL	0	NULL	lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One issue that has received little consideration so far is whether the hippocampus can function normally in the presence of a lesion to perirhinal cortex that produces noticeable memory impairments .
	manualset3
122948	6	404235	13	NULL	NULL	0	NULL	perirhinal cortex 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	One issue that has received little consideration so far is whether the hippocampus can function normally in the presence of a lesion to perirhinal cortex that produces noticeable memory impairments .
	manualset3
122949	7	404235	13	NULL	NULL	0	NULL	noticeable memory impairments	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One issue that has received little consideration so far is whether the hippocampus can function normally in the presence of a lesion to perirhinal cortex that produces noticeable memory impairments .
	manualset3
123028	8	404235	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One issue that has received little consideration so far is whether the hippocampus can function normally in the presence of a lesion to perirhinal cortex that produces noticeable memory impairments .
	manualset3
122950	1	404236	13	NULL	NULL	0	NULL	mechanism 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One mechanism by which mammalian cells regulate the uptake of glucose is the number of glucose transporter proteins ( GLUT ) present at the plasma membrane .
	manualset3
122951	2	404236	13	NULL	NULL	0	NULL	mammalian cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	One mechanism by which mammalian cells regulate the uptake of glucose is the number of glucose transporter proteins ( GLUT ) present at the plasma membrane .
	manualset3
122952	3	404236	13	NULL	NULL	0	NULL	uptake of glucose	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One mechanism by which mammalian cells regulate the uptake of glucose is the number of glucose transporter proteins ( GLUT ) present at the plasma membrane .
	manualset3
122953	4	404236	13	NULL	NULL	0	NULL	number of glucose transporter proteins ( GLUT )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One mechanism by which mammalian cells regulate the uptake of glucose is the number of glucose transporter proteins ( GLUT ) present at the plasma membrane .
	manualset3
122954	5	404236	13	NULL	NULL	0	NULL	plasma membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	One mechanism by which mammalian cells regulate the uptake of glucose is the number of glucose transporter proteins ( GLUT ) present at the plasma membrane .
	manualset3
123027	6	404236	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One mechanism by which mammalian cells regulate the uptake of glucose is the number of glucose transporter proteins ( GLUT ) present at the plasma membrane .
	manualset3
122955	1	404237	13	NULL	NULL	0	NULL	mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One mechanism of this restriction is deamination of cytidines to uridines in ( - ) strand DNA , resulting in hypermutation of guanosines to adenosines in viral ( + ) strands .
	manualset3
122956	2	404237	13	NULL	NULL	0	NULL	restriction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One mechanism of this restriction is deamination of cytidines to uridines in ( - ) strand DNA , resulting in hypermutation of guanosines to adenosines in viral ( + ) strands .
	manualset3
122957	3	404237	13	NULL	NULL	0	NULL	deamination 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One mechanism of this restriction is deamination of cytidines to uridines in ( - ) strand DNA , resulting in hypermutation of guanosines to adenosines in viral ( + ) strands .
	manualset3
122958	4	404237	13	NULL	NULL	0	NULL	cytidines	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	One mechanism of this restriction is deamination of cytidines to uridines in ( - ) strand DNA , resulting in hypermutation of guanosines to adenosines in viral ( + ) strands .
	manualset3
122959	5	404237	13	NULL	NULL	0	NULL	uridines	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	One mechanism of this restriction is deamination of cytidines to uridines in ( - ) strand DNA , resulting in hypermutation of guanosines to adenosines in viral ( + ) strands .
	manualset3
122960	6	404237	13	NULL	NULL	0	NULL	( - ) strand DNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	One mechanism of this restriction is deamination of cytidines to uridines in ( - ) strand DNA , resulting in hypermutation of guanosines to adenosines in viral ( + ) strands .
	manualset3
122961	7	404237	13	NULL	NULL	0	NULL	hypermutation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One mechanism of this restriction is deamination of cytidines to uridines in ( - ) strand DNA , resulting in hypermutation of guanosines to adenosines in viral ( + ) strands .
	manualset3
122962	8	404237	13	NULL	NULL	0	NULL	guanosines 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	One mechanism of this restriction is deamination of cytidines to uridines in ( - ) strand DNA , resulting in hypermutation of guanosines to adenosines in viral ( + ) strands .
	manualset3
122963	9	404237	13	NULL	NULL	0	NULL	adenosines	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	One mechanism of this restriction is deamination of cytidines to uridines in ( - ) strand DNA , resulting in hypermutation of guanosines to adenosines in viral ( + ) strands .
	manualset3
122964	10	404237	13	NULL	NULL	0	NULL	viral ( + ) strands	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	One mechanism of this restriction is deamination of cytidines to uridines in ( - ) strand DNA , resulting in hypermutation of guanosines to adenosines in viral ( + ) strands .
	manualset3
123026	11	404237	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One mechanism of this restriction is deamination of cytidines to uridines in ( - ) strand DNA , resulting in hypermutation of guanosines to adenosines in viral ( + ) strands .
	manualset3
122967	1	404238	13	NULL	NULL	0	NULL	mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One mechanism through which sleep loss may contribute to depressive symptomatology is by affecting hippocampal function .
	manualset3
122969	2	404238	13	NULL	NULL	0	NULL	sleep loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One mechanism through which sleep loss may contribute to depressive symptomatology is by affecting hippocampal function .
	manualset3
122971	3	404238	13	NULL	NULL	0	NULL	depressive symptomatology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One mechanism through which sleep loss may contribute to depressive symptomatology is by affecting hippocampal function .
	manualset3
122972	4	404238	13	NULL	NULL	0	NULL	hippocampal function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One mechanism through which sleep loss may contribute to depressive symptomatology is by affecting hippocampal function .
	manualset3
123025	5	404238	13	NULL	NULL	0	NULL	One 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One mechanism through which sleep loss may contribute to depressive symptomatology is by affecting hippocampal function .
	manualset3
122974	1	404239	13	NULL	NULL	0	NULL	family of arginine-phenylalanine amide peptides 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	One member of this family of arginine-phenylalanine amide peptides , KP-54 , was subsequently identified as the natural ligand for the G-protein coupled receptor-54 ( GPR54 ) .
	manualset3
122976	2	404239	13	NULL	NULL	0	NULL	One member	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	One member of this family of arginine-phenylalanine amide peptides , KP-54 , was subsequently identified as the natural ligand for the G-protein coupled receptor-54 ( GPR54 ) .
	manualset3
122979	3	404239	13	NULL	NULL	0	NULL	KP-54	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	One member of this family of arginine-phenylalanine amide peptides , KP-54 , was subsequently identified as the natural ligand for the G-protein coupled receptor-54 ( GPR54 ) .
	manualset3
122981	4	404239	13	NULL	NULL	0	NULL	natural ligand 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	One member of this family of arginine-phenylalanine amide peptides , KP-54 , was subsequently identified as the natural ligand for the G-protein coupled receptor-54 ( GPR54 ) .
	manualset3
122982	5	404239	13	NULL	NULL	0	NULL	G-protein coupled receptor-54 ( GPR54 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One member of this family of arginine-phenylalanine amide peptides , KP-54 , was subsequently identified as the natural ligand for the G-protein coupled receptor-54 ( GPR54 ) .
	manualset3
122984	1	404240	13	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A difference in the adhesive capacity of periurethral cells of infection-prone and healthy individuals was most evident at concentrations of 2.5 x 10 ( 9 ) bacteria/ml .
	manualset3
122985	2	404240	13	NULL	NULL	0	NULL	adhesive capacity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A difference in the adhesive capacity of periurethral cells of infection-prone and healthy individuals was most evident at concentrations of 2.5 x 10 ( 9 ) bacteria/ml .
	manualset3
122986	3	404240	13	NULL	NULL	0	NULL	periurethral cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A difference in the adhesive capacity of periurethral cells of infection-prone and healthy individuals was most evident at concentrations of 2.5 x 10 ( 9 ) bacteria/ml .
	manualset3
122987	4	404240	13	NULL	NULL	0	NULL	infection-prone individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A difference in the adhesive capacity of periurethral cells of infection-prone and healthy individuals was most evident at concentrations of 2.5 x 10 ( 9 ) bacteria/ml .
	manualset3
122988	5	404240	13	NULL	NULL	0	NULL	healthy individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A difference in the adhesive capacity of periurethral cells of infection-prone and healthy individuals was most evident at concentrations of 2.5 x 10 ( 9 ) bacteria/ml .
	manualset3
122989	6	404240	13	NULL	NULL	0	NULL	concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A difference in the adhesive capacity of periurethral cells of infection-prone and healthy individuals was most evident at concentrations of 2.5 x 10 ( 9 ) bacteria/ml .
	manualset3
122990	7	404240	13	NULL	NULL	0	NULL	2.5 x 10 ( 9 ) bacteria/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A difference in the adhesive capacity of periurethral cells of infection-prone and healthy individuals was most evident at concentrations of 2.5 x 10 ( 9 ) bacteria/ml .
	manualset3
122992	1	404241	13	NULL	NULL	0	NULL	One milligram	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One milligram of the FPLC-fractionated robinin generated an ORAC value of 5.15 + / - 2.00 micromol/mg of Trolox , whereas 1 mg of pure robinin generated an ORAC value of 12.34 + / - 0.45 micromol/mg of Trolox .
	manualset3
122993	2	404241	13	NULL	NULL	0	NULL	FPLC-fractionated robinin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	One milligram of the FPLC-fractionated robinin generated an ORAC value of 5.15 + / - 2.00 micromol/mg of Trolox , whereas 1 mg of pure robinin generated an ORAC value of 12.34 + / - 0.45 micromol/mg of Trolox .
	manualset3
122994	3	404241	13	NULL	NULL	0	NULL	ORAC value	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One milligram of the FPLC-fractionated robinin generated an ORAC value of 5.15 + / - 2.00 micromol/mg of Trolox , whereas 1 mg of pure robinin generated an ORAC value of 12.34 + / - 0.45 micromol/mg of Trolox .
	manualset3
122995	4	404241	13	NULL	NULL	0	NULL	5.15 + / - 2.00 micromol/mg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One milligram of the FPLC-fractionated robinin generated an ORAC value of 5.15 + / - 2.00 micromol/mg of Trolox , whereas 1 mg of pure robinin generated an ORAC value of 12.34 + / - 0.45 micromol/mg of Trolox .
	manualset3
122996	5	404241	13	NULL	NULL	0	NULL	Trolox	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	One milligram of the FPLC-fractionated robinin generated an ORAC value of 5.15 + / - 2.00 micromol/mg of Trolox , whereas 1 mg of pure robinin generated an ORAC value of 12.34 + / - 0.45 micromol/mg of Trolox .
	manualset3
122997	6	404241	13	NULL	NULL	NULL	NULL	1 mg 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	One milligram of the FPLC-fractionated robinin generated an ORAC value of 5.15 + / - 2.00 micromol/mg of Trolox , whereas 1 mg of pure robinin generated an ORAC value of 12.34 + / - 0.45 micromol/mg of Trolox .
	manualset3
122998	7	404241	13	NULL	NULL	0	NULL	robinin 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	One milligram of the FPLC-fractionated robinin generated an ORAC value of 5.15 + / - 2.00 micromol/mg of Trolox , whereas 1 mg of pure robinin generated an ORAC value of 12.34 + / - 0.45 micromol/mg of Trolox .
	manualset3
122999	8	404241	13	NULL	NULL	0	NULL	ORAC value 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One milligram of the FPLC-fractionated robinin generated an ORAC value of 5.15 + / - 2.00 micromol/mg of Trolox , whereas 1 mg of pure robinin generated an ORAC value of 12.34 + / - 0.45 micromol/mg of Trolox .
	manualset3
123000	9	404241	13	NULL	NULL	0	NULL	12.34 + / - 0.45 micromol/mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One milligram of the FPLC-fractionated robinin generated an ORAC value of 5.15 + / - 2.00 micromol/mg of Trolox , whereas 1 mg of pure robinin generated an ORAC value of 12.34 + / - 0.45 micromol/mg of Trolox .
	manualset3
123001	10	404241	13	NULL	NULL	0	NULL	Trolox	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	One milligram of the FPLC-fractionated robinin generated an ORAC value of 5.15 + / - 2.00 micromol/mg of Trolox , whereas 1 mg of pure robinin generated an ORAC value of 12.34 + / - 0.45 micromol/mg of Trolox .
	manualset3
123002	1	404242	13	NULL	NULL	0	NULL	mixture	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	One mixture of structurally congeneric phenylureas and one mixture of non-congeneric PSII inhibitors were tested .
	manualset3
123003	2	404242	13	NULL	NULL	0	NULL	congeneric phenylureas	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	One mixture of structurally congeneric phenylureas and one mixture of non-congeneric PSII inhibitors were tested .
	manualset3
123004	3	404242	13	NULL	NULL	0	NULL	mixture	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	One mixture of structurally congeneric phenylureas and one mixture of non-congeneric PSII inhibitors were tested .
	manualset3
123005	4	404242	13	NULL	NULL	0	NULL	non-congeneric PSII inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	One mixture of structurally congeneric phenylureas and one mixture of non-congeneric PSII inhibitors were tested .
	manualset3
123023	5	404242	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One mixture of structurally congeneric phenylureas and one mixture of non-congeneric PSII inhibitors were tested .
	manualset3
123024	6	404242	13	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One mixture of structurally congeneric phenylureas and one mixture of non-congeneric PSII inhibitors were tested .
	manualset3
123006	1	404243	13	NULL	NULL	0	NULL	One month	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	One month later the patient was readmitted with systemic disease and cardiac insufficiency .
	manualset3
123007	2	404243	13	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	One month later the patient was readmitted with systemic disease and cardiac insufficiency .
	manualset3
123008	3	404243	13	NULL	NULL	0	NULL	systemic disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	One month later the patient was readmitted with systemic disease and cardiac insufficiency .
	manualset3
123009	4	404243	13	NULL	NULL	0	NULL	cardiac insufficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One month later the patient was readmitted with systemic disease and cardiac insufficiency .
	manualset3
123010	1	404244	13	NULL	NULL	0	NULL	mutation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One mutation was identified in DNA isolated from prostatic cancer tissue , and the mutation was also detected in the leukocyte DNA of the patient and his offspring .
	manualset3
123011	2	404244	13	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	One mutation was identified in DNA isolated from prostatic cancer tissue , and the mutation was also detected in the leukocyte DNA of the patient and his offspring .
	manualset3
123012	3	404244	13	NULL	NULL	0	NULL	prostatic cancer tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	One mutation was identified in DNA isolated from prostatic cancer tissue , and the mutation was also detected in the leukocyte DNA of the patient and his offspring .
	manualset3
123013	4	404244	13	NULL	NULL	0	NULL	mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One mutation was identified in DNA isolated from prostatic cancer tissue , and the mutation was also detected in the leukocyte DNA of the patient and his offspring .
	manualset3
123014	5	404244	13	NULL	NULL	0	NULL	leukocyte DNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	One mutation was identified in DNA isolated from prostatic cancer tissue , and the mutation was also detected in the leukocyte DNA of the patient and his offspring .
	manualset3
123015	6	404244	13	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	One mutation was identified in DNA isolated from prostatic cancer tissue , and the mutation was also detected in the leukocyte DNA of the patient and his offspring .
	manualset3
123016	7	404244	13	NULL	NULL	0	NULL	offspring	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	One mutation was identified in DNA isolated from prostatic cancer tissue , and the mutation was also detected in the leukocyte DNA of the patient and his offspring .
	manualset3
123022	8	404244	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One mutation was identified in DNA isolated from prostatic cancer tissue , and the mutation was also detected in the leukocyte DNA of the patient and his offspring .
	manualset3
123017	1	404245	13	NULL	NULL	0	NULL	17 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the 17 patients without angiographic TI was diagnosed as mild TI by MRI ( specificity = 94 % ) .
	manualset3
123018	2	404245	13	NULL	NULL	0	NULL	angiographic TI	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the 17 patients without angiographic TI was diagnosed as mild TI by MRI ( specificity = 94 % ) .
	manualset3
123019	3	404245	13	NULL	NULL	0	NULL	mild TI 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the 17 patients without angiographic TI was diagnosed as mild TI by MRI ( specificity = 94 % ) .
	manualset3
123020	4	404245	13	NULL	NULL	0	NULL	MRI	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the 17 patients without angiographic TI was diagnosed as mild TI by MRI ( specificity = 94 % ) .
	manualset3
123021	5	404245	13	NULL	NULL	0	NULL	specificity = 94 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the 17 patients without angiographic TI was diagnosed as mild TI by MRI ( specificity = 94 % ) .
	manualset3
123043	1	404246	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the CARD-containing proteins , TUCAN ( CARD8 ) , was reported previously as an antiapoptotic protein with a molecular weight of 48 kDa , which was up-regulated in colon cancer cells .
	manualset3
123044	2	404246	13	NULL	NULL	0	NULL	CARD-containing proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the CARD-containing proteins , TUCAN ( CARD8 ) , was reported previously as an antiapoptotic protein with a molecular weight of 48 kDa , which was up-regulated in colon cancer cells .
	manualset3
123045	3	404246	13	NULL	NULL	0	NULL	TUCAN ( CARD8 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the CARD-containing proteins , TUCAN ( CARD8 ) , was reported previously as an antiapoptotic protein with a molecular weight of 48 kDa , which was up-regulated in colon cancer cells .
	manualset3
123046	4	404246	13	NULL	NULL	0	NULL	antiapoptotic protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the CARD-containing proteins , TUCAN ( CARD8 ) , was reported previously as an antiapoptotic protein with a molecular weight of 48 kDa , which was up-regulated in colon cancer cells .
	manualset3
123047	5	404246	13	NULL	NULL	0	NULL	molecular weight of 48 kDa	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the CARD-containing proteins , TUCAN ( CARD8 ) , was reported previously as an antiapoptotic protein with a molecular weight of 48 kDa , which was up-regulated in colon cancer cells .
	manualset3
123048	6	404246	13	NULL	NULL	0	NULL	colon cancer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the CARD-containing proteins , TUCAN ( CARD8 ) , was reported previously as an antiapoptotic protein with a molecular weight of 48 kDa , which was up-regulated in colon cancer cells .
	manualset3
123049	1	404247	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the IL-9-regulated genes isolated by this approach turned out to encode a 180-amino acid long protein , including a potential signal peptide , and showing 22 % amino acid identity with IL-10 .
	manualset3
123050	2	404247	13	NULL	NULL	0	NULL	IL-9-regulated genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the IL-9-regulated genes isolated by this approach turned out to encode a 180-amino acid long protein , including a potential signal peptide , and showing 22 % amino acid identity with IL-10 .
	manualset3
123051	3	404247	13	NULL	NULL	0	NULL	approach	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the IL-9-regulated genes isolated by this approach turned out to encode a 180-amino acid long protein , including a potential signal peptide , and showing 22 % amino acid identity with IL-10 .
	manualset3
123052	4	404247	13	NULL	NULL	0	NULL	180-amino acid long protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the IL-9-regulated genes isolated by this approach turned out to encode a 180-amino acid long protein , including a potential signal peptide , and showing 22 % amino acid identity with IL-10 .
	manualset3
123053	5	404247	13	NULL	NULL	0	NULL	potential signal peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the IL-9-regulated genes isolated by this approach turned out to encode a 180-amino acid long protein , including a potential signal peptide , and showing 22 % amino acid identity with IL-10 .
	manualset3
123054	6	404247	13	NULL	NULL	0	NULL	22 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the IL-9-regulated genes isolated by this approach turned out to encode a 180-amino acid long protein , including a potential signal peptide , and showing 22 % amino acid identity with IL-10 .
	manualset3
123055	7	404247	13	NULL	NULL	0	NULL	amino acid identity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the IL-9-regulated genes isolated by this approach turned out to encode a 180-amino acid long protein , including a potential signal peptide , and showing 22 % amino acid identity with IL-10 .
	manualset3
123056	8	404247	13	NULL	NULL	0	NULL	IL-10	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the IL-9-regulated genes isolated by this approach turned out to encode a 180-amino acid long protein , including a potential signal peptide , and showing 22 % amino acid identity with IL-10 .
	manualset3
123057	1	404248	13	NULL	NULL	0	NULL	One 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the approaches was to add the dried plant of Leguminosae ( saponin ) or tea flower ( saponin ) , when `` BANCHA '' was decorted .
	manualset3
123058	2	404248	13	NULL	NULL	0	NULL	approaches	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the approaches was to add the dried plant of Leguminosae ( saponin ) or tea flower ( saponin ) , when `` BANCHA '' was decorted .
	manualset3
123059	3	404248	13	NULL	NULL	0	NULL	 plant of Leguminosae ( saponin )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the approaches was to add the dried plant of Leguminosae ( saponin ) or tea flower ( saponin ) , when `` BANCHA '' was decorted .
	manualset3
123060	4	404248	13	NULL	NULL	0	NULL	tea flower ( saponin )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the approaches was to add the dried plant of Leguminosae ( saponin ) or tea flower ( saponin ) , when `` BANCHA '' was decorted .
	manualset3
123061	5	404248	13	NULL	NULL	0	NULL	BANCHA	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the approaches was to add the dried plant of Leguminosae ( saponin ) or tea flower ( saponin ) , when `` BANCHA '' was decorted .
	manualset3
123062	1	404249	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the cases with ketoacidosis had peritonitis and pancreatitis .
	manualset3
123063	2	404249	13	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the cases with ketoacidosis had peritonitis and pancreatitis .
	manualset3
123064	3	404249	13	NULL	NULL	0	NULL	ketoacidosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the cases with ketoacidosis had peritonitis and pancreatitis .
	manualset3
123065	4	404249	13	NULL	NULL	0	NULL	peritonitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the cases with ketoacidosis had peritonitis and pancreatitis .
	manualset3
123066	5	404249	13	NULL	NULL	0	NULL	pancreatitis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the cases with ketoacidosis had peritonitis and pancreatitis .
	manualset3
123067	1	404250	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the genes , cpn60 .1 , although actively transcribed , is not expressed to detectable levels of protein in cultured L. donovani .
	manualset3
123068	2	404250	13	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the genes , cpn60 .1 , although actively transcribed , is not expressed to detectable levels of protein in cultured L. donovani .
	manualset3
123069	3	404250	13	NULL	NULL	0	NULL	cpn60 .1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the genes , cpn60 .1 , although actively transcribed , is not expressed to detectable levels of protein in cultured L. donovani .
	manualset3
123070	4	404250	13	NULL	NULL	0	NULL	levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the genes , cpn60 .1 , although actively transcribed , is not expressed to detectable levels of protein in cultured L. donovani .
	manualset3
123071	5	404250	13	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the genes , cpn60 .1 , although actively transcribed , is not expressed to detectable levels of protein in cultured L. donovani .
	manualset3
123072	6	404250	13	NULL	NULL	0	NULL	L. donovani	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the genes , cpn60 .1 , although actively transcribed , is not expressed to detectable levels of protein in cultured L. donovani .
	manualset3
123073	1	404251	13	NULL	NULL	0	NULL	One 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the key viral regulatory proteins , Tat , which is released by infected cells , can be taken up by various uninfected cells including neurons and by dysregulating several biological events induces cell injury and death .
	manualset3
123074	2	404251	13	NULL	NULL	0	NULL	key viral regulatory proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the key viral regulatory proteins , Tat , which is released by infected cells , can be taken up by various uninfected cells including neurons and by dysregulating several biological events induces cell injury and death .
	manualset3
123075	3	404251	13	NULL	NULL	0	NULL	Tat	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the key viral regulatory proteins , Tat , which is released by infected cells , can be taken up by various uninfected cells including neurons and by dysregulating several biological events induces cell injury and death .
	manualset3
123076	4	404251	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the key viral regulatory proteins , Tat , which is released by infected cells , can be taken up by various uninfected cells including neurons and by dysregulating several biological events induces cell injury and death .
	manualset3
123077	5	404251	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the key viral regulatory proteins , Tat , which is released by infected cells , can be taken up by various uninfected cells including neurons and by dysregulating several biological events induces cell injury and death .
	manualset3
123078	6	404251	13	NULL	NULL	0	NULL	neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the key viral regulatory proteins , Tat , which is released by infected cells , can be taken up by various uninfected cells including neurons and by dysregulating several biological events induces cell injury and death .
	manualset3
123079	7	404251	13	NULL	NULL	0	NULL	biological events	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the key viral regulatory proteins , Tat , which is released by infected cells , can be taken up by various uninfected cells including neurons and by dysregulating several biological events induces cell injury and death .
	manualset3
123080	8	404251	13	NULL	NULL	0	NULL	cell injury	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the key viral regulatory proteins , Tat , which is released by infected cells , can be taken up by various uninfected cells including neurons and by dysregulating several biological events induces cell injury and death .
	manualset3
123081	9	404251	13	NULL	NULL	0	NULL	death 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the key viral regulatory proteins , Tat , which is released by infected cells , can be taken up by various uninfected cells including neurons and by dysregulating several biological events induces cell injury and death .
	manualset3
123082	1	404252	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the main approaches towards inhibiting its activity is the development of phosphopetides or peptidomimetics that competitively bind to the SH2 domain of Stat3 .
	manualset3
123083	2	404252	13	NULL	NULL	0	NULL	approaches	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the main approaches towards inhibiting its activity is the development of phosphopetides or peptidomimetics that competitively bind to the SH2 domain of Stat3 .
	manualset3
123084	3	404252	13	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the main approaches towards inhibiting its activity is the development of phosphopetides or peptidomimetics that competitively bind to the SH2 domain of Stat3 .
	manualset3
123085	4	404252	13	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the main approaches towards inhibiting its activity is the development of phosphopetides or peptidomimetics that competitively bind to the SH2 domain of Stat3 .
	manualset3
123086	5	404252	13	NULL	NULL	0	NULL	phosphopetides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the main approaches towards inhibiting its activity is the development of phosphopetides or peptidomimetics that competitively bind to the SH2 domain of Stat3 .
	manualset3
123087	6	404252	13	NULL	NULL	0	NULL	peptidomimetics	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the main approaches towards inhibiting its activity is the development of phosphopetides or peptidomimetics that competitively bind to the SH2 domain of Stat3 .
	manualset3
123088	7	404252	13	NULL	NULL	0	NULL	SH2 domain of Stat3	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the main approaches towards inhibiting its activity is the development of phosphopetides or peptidomimetics that competitively bind to the SH2 domain of Stat3 .
	manualset3
123112	1	404253	13	NULL	NULL	0	NULL	main tasks	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the main tasks of contemporary medical anthropology is to discover the devices and processes that connect these two spheres -- the states of health of the person 's body and of the social body/group of which he is a part -- through the origin , development and experience of illness .
	manualset3
123113	2	404253	13	NULL	NULL	0	NULL	medical anthropology 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the main tasks of contemporary medical anthropology is to discover the devices and processes that connect these two spheres -- the states of health of the person 's body and of the social body/group of which he is a part -- through the origin , development and experience of illness .
	manualset3
123114	3	404253	13	NULL	NULL	0	NULL	devices	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the main tasks of contemporary medical anthropology is to discover the devices and processes that connect these two spheres -- the states of health of the person 's body and of the social body/group of which he is a part -- through the origin , development and experience of illness .
	manualset3
123115	4	404253	13	NULL	NULL	0	NULL	processes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the main tasks of contemporary medical anthropology is to discover the devices and processes that connect these two spheres -- the states of health of the person 's body and of the social body/group of which he is a part -- through the origin , development and experience of illness .
	manualset3
123118	5	404253	13	NULL	NULL	0	NULL	two spheres	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the main tasks of contemporary medical anthropology is to discover the devices and processes that connect these two spheres -- the states of health of the person 's body and of the social body/group of which he is a part -- through the origin , development and experience of illness .
	manualset3
123119	6	404253	13	NULL	NULL	0	NULL	states of health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the main tasks of contemporary medical anthropology is to discover the devices and processes that connect these two spheres -- the states of health of the person 's body and of the social body/group of which he is a part -- through the origin , development and experience of illness .
	manualset3
123120	7	404253	13	NULL	NULL	0	NULL	person 's body	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the main tasks of contemporary medical anthropology is to discover the devices and processes that connect these two spheres -- the states of health of the person 's body and of the social body/group of which he is a part -- through the origin , development and experience of illness .
	manualset3
123121	8	404253	13	NULL	NULL	0	NULL	social body/group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the main tasks of contemporary medical anthropology is to discover the devices and processes that connect these two spheres -- the states of health of the person 's body and of the social body/group of which he is a part -- through the origin , development and experience of illness .
	manualset3
123123	9	404253	13	NULL	NULL	0	NULL	origin of illness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the main tasks of contemporary medical anthropology is to discover the devices and processes that connect these two spheres -- the states of health of the person 's body and of the social body/group of which he is a part -- through the origin , development and experience of illness .
	manualset3
123124	10	404253	13	NULL	NULL	0	NULL	development of illness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the main tasks of contemporary medical anthropology is to discover the devices and processes that connect these two spheres -- the states of health of the person 's body and of the social body/group of which he is a part -- through the origin , development and experience of illness .
	manualset3
123125	11	404253	13	NULL	NULL	0	NULL	experience of illness 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the main tasks of contemporary medical anthropology is to discover the devices and processes that connect these two spheres -- the states of health of the person 's body and of the social body/group of which he is a part -- through the origin , development and experience of illness .
	manualset3
123126	1	404254	13	NULL	NULL	0	NULL	adverse drug reactions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the most important adverse drug reactions that physicians encounter is the life - and limb-threatening prothrombotic syndrome known as heparin-induced thrombocytopenia ( HIT ) .
	manualset3
123127	2	404254	13	NULL	NULL	0	NULL	physicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the most important adverse drug reactions that physicians encounter is the life - and limb-threatening prothrombotic syndrome known as heparin-induced thrombocytopenia ( HIT ) .
	manualset3
123128	3	404254	13	NULL	NULL	0	NULL	life - threatening prothrombotic syndrome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the most important adverse drug reactions that physicians encounter is the life - and limb-threatening prothrombotic syndrome known as heparin-induced thrombocytopenia ( HIT ) .
	manualset3
123129	4	404254	13	NULL	NULL	0	NULL	limb-threatening prothrombotic syndrome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the most important adverse drug reactions that physicians encounter is the life - and limb-threatening prothrombotic syndrome known as heparin-induced thrombocytopenia ( HIT ) .
	manualset3
123132	5	404254	13	NULL	NULL	0	NULL	heparin-induced thrombocytopenia ( HIT )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the most important adverse drug reactions that physicians encounter is the life - and limb-threatening prothrombotic syndrome known as heparin-induced thrombocytopenia ( HIT ) .
	manualset3
123136	6	404254	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the most important adverse drug reactions that physicians encounter is the life - and limb-threatening prothrombotic syndrome known as heparin-induced thrombocytopenia ( HIT ) .
	manualset3
123137	1	404255	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the most striking features of the injured mature peripheral nervous system is the ability to regenerate .
	manualset3
123138	2	404255	13	NULL	NULL	0	NULL	features	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the most striking features of the injured mature peripheral nervous system is the ability to regenerate .
	manualset3
123139	3	404255	13	NULL	NULL	0	NULL	mature peripheral nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the most striking features of the injured mature peripheral nervous system is the ability to regenerate .
	manualset3
123140	4	404255	13	NULL	NULL	0	NULL	ability 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the most striking features of the injured mature peripheral nervous system is the ability to regenerate .
	manualset3
123142	1	404256	13	NULL	NULL	0	NULL	new inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the new inhibitors is highly effective against an atovaquone resistant Plasmodium and illustrates the type of modification to the hydroxy-naphthoquinone ring of atovaquone that might mitigate drug resistance .
	manualset3
123144	2	404256	13	NULL	NULL	0	NULL	atovaquone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the new inhibitors is highly effective against an atovaquone resistant Plasmodium and illustrates the type of modification to the hydroxy-naphthoquinone ring of atovaquone that might mitigate drug resistance .
	manualset3
123145	3	404256	13	NULL	NULL	0	NULL	Plasmodium	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the new inhibitors is highly effective against an atovaquone resistant Plasmodium and illustrates the type of modification to the hydroxy-naphthoquinone ring of atovaquone that might mitigate drug resistance .
	manualset3
123146	4	404256	13	NULL	NULL	0	NULL	type of modification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the new inhibitors is highly effective against an atovaquone resistant Plasmodium and illustrates the type of modification to the hydroxy-naphthoquinone ring of atovaquone that might mitigate drug resistance .
	manualset3
123147	5	404256	13	NULL	NULL	0	NULL	hydroxy-naphthoquinone ring 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the new inhibitors is highly effective against an atovaquone resistant Plasmodium and illustrates the type of modification to the hydroxy-naphthoquinone ring of atovaquone that might mitigate drug resistance .
	manualset3
123149	6	404256	13	NULL	NULL	0	NULL	atovaquone 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the new inhibitors is highly effective against an atovaquone resistant Plasmodium and illustrates the type of modification to the hydroxy-naphthoquinone ring of atovaquone that might mitigate drug resistance .
	manualset3
123151	7	404256	13	NULL	NULL	0	NULL	drug resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the new inhibitors is highly effective against an atovaquone resistant Plasmodium and illustrates the type of modification to the hydroxy-naphthoquinone ring of atovaquone that might mitigate drug resistance .
	manualset3
123164	8	404256	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the new inhibitors is highly effective against an atovaquone resistant Plasmodium and illustrates the type of modification to the hydroxy-naphthoquinone ring of atovaquone that might mitigate drug resistance .
	manualset3
123159	1	404257	13	NULL	NULL	0	NULL	 pathological hallmarks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the pathological hallmarks of LD is the presence of cytoplasmic PAS + polyglucosan inclusions called Lafora bodies ( LBs ) .
	manualset3
123160	2	404257	13	NULL	NULL	0	NULL	LD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the pathological hallmarks of LD is the presence of cytoplasmic PAS + polyglucosan inclusions called Lafora bodies ( LBs ) .
	manualset3
123161	3	404257	13	NULL	NULL	0	NULL	presence of cytoplasmic PAS + polyglucosan inclusions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the pathological hallmarks of LD is the presence of cytoplasmic PAS + polyglucosan inclusions called Lafora bodies ( LBs ) .
	manualset3
123162	4	404257	13	NULL	NULL	0	NULL	Lafora bodies ( LBs )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the pathological hallmarks of LD is the presence of cytoplasmic PAS + polyglucosan inclusions called Lafora bodies ( LBs ) .
	manualset3
123163	5	404257	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the pathological hallmarks of LD is the presence of cytoplasmic PAS + polyglucosan inclusions called Lafora bodies ( LBs ) .
	manualset3
123165	1	404258	13	NULL	NULL	0	NULL	One 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the patient 's C1-INH gene alleles was revealed to have at least a 17-kb-length deletion including exons 5-8 .
	manualset3
123166	2	404258	13	NULL	NULL	0	NULL	patient 's 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the patient 's C1-INH gene alleles was revealed to have at least a 17-kb-length deletion including exons 5-8 .
	manualset3
123167	3	404258	13	NULL	NULL	0	NULL	C1-INH gene alleles 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the patient 's C1-INH gene alleles was revealed to have at least a 17-kb-length deletion including exons 5-8 .
	manualset3
123168	4	404258	13	NULL	NULL	0	NULL	17-kb-length	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the patient 's C1-INH gene alleles was revealed to have at least a 17-kb-length deletion including exons 5-8 .
	manualset3
123169	5	404258	13	NULL	NULL	0	NULL	deletion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the patient 's C1-INH gene alleles was revealed to have at least a 17-kb-length deletion including exons 5-8 .
	manualset3
123170	6	404258	13	NULL	NULL	0	NULL	exons 5-8	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the patient 's C1-INH gene alleles was revealed to have at least a 17-kb-length deletion including exons 5-8 .
	manualset3
123171	1	404259	13	NULL	NULL	0	NULL	One 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the possible mechanisms by which resveratrol affects these disease states is by affecting the cellular signaling network involving protein kinase C alpha ( PKC ) .
	manualset3
123174	2	404259	13	NULL	NULL	0	NULL	mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the possible mechanisms by which resveratrol affects these disease states is by affecting the cellular signaling network involving protein kinase C alpha ( PKC ) .
	manualset3
123175	3	404259	13	NULL	NULL	0	NULL	resveratrol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the possible mechanisms by which resveratrol affects these disease states is by affecting the cellular signaling network involving protein kinase C alpha ( PKC ) .
	manualset3
123177	4	404259	13	NULL	NULL	0	NULL	disease states 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the possible mechanisms by which resveratrol affects these disease states is by affecting the cellular signaling network involving protein kinase C alpha ( PKC ) .
	manualset3
123178	5	404259	13	NULL	NULL	0	NULL	cellular signaling network	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the possible mechanisms by which resveratrol affects these disease states is by affecting the cellular signaling network involving protein kinase C alpha ( PKC ) .
	manualset3
123179	6	404259	13	NULL	NULL	0	NULL	protein kinase C alpha ( PKC )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the possible mechanisms by which resveratrol affects these disease states is by affecting the cellular signaling network involving protein kinase C alpha ( PKC ) .
	manualset3
123180	1	404260	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the reasons may be the increased production and role of nitric oxide in pulmonary artery tone .
	manualset3
123181	2	404260	13	NULL	NULL	0	NULL	reasons 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the reasons may be the increased production and role of nitric oxide in pulmonary artery tone .
	manualset3
123182	3	404260	13	NULL	NULL	0	NULL	production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the reasons may be the increased production and role of nitric oxide in pulmonary artery tone .
	manualset3
123183	4	404260	13	NULL	NULL	0	NULL	role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the reasons may be the increased production and role of nitric oxide in pulmonary artery tone .
	manualset3
123184	5	404260	13	NULL	NULL	0	NULL	nitric oxide 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the reasons may be the increased production and role of nitric oxide in pulmonary artery tone .
	manualset3
123185	6	404260	13	NULL	NULL	0	NULL	pulmonary artery tone 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the reasons may be the increased production and role of nitric oxide in pulmonary artery tone .
	manualset3
123188	1	404261	13	NULL	NULL	0	NULL	recent breakthrough studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the recent breakthrough studies in TOR signaling resulted in the identification of the tuberous sclerosis complex gene products , TSC1 and TSC2 , as negative regulators for TOR signaling .
	manualset3
123189	2	404261	13	NULL	NULL	0	NULL	TOR signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the recent breakthrough studies in TOR signaling resulted in the identification of the tuberous sclerosis complex gene products , TSC1 and TSC2 , as negative regulators for TOR signaling .
	manualset3
123190	3	404261	13	NULL	NULL	0	NULL	identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the recent breakthrough studies in TOR signaling resulted in the identification of the tuberous sclerosis complex gene products , TSC1 and TSC2 , as negative regulators for TOR signaling .
	manualset3
123191	4	404261	13	NULL	NULL	0	NULL	tuberous sclerosis complex gene products	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the recent breakthrough studies in TOR signaling resulted in the identification of the tuberous sclerosis complex gene products , TSC1 and TSC2 , as negative regulators for TOR signaling .
	manualset3
123192	5	404261	13	NULL	NULL	0	NULL	TSC1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the recent breakthrough studies in TOR signaling resulted in the identification of the tuberous sclerosis complex gene products , TSC1 and TSC2 , as negative regulators for TOR signaling .
	manualset3
123193	6	404261	13	NULL	NULL	0	NULL	TSC2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the recent breakthrough studies in TOR signaling resulted in the identification of the tuberous sclerosis complex gene products , TSC1 and TSC2 , as negative regulators for TOR signaling .
	manualset3
123194	7	404261	13	NULL	NULL	0	NULL	negative regulators 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the recent breakthrough studies in TOR signaling resulted in the identification of the tuberous sclerosis complex gene products , TSC1 and TSC2 , as negative regulators for TOR signaling .
	manualset3
123195	8	404261	13	NULL	NULL	0	NULL	TOR signaling 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the recent breakthrough studies in TOR signaling resulted in the identification of the tuberous sclerosis complex gene products , TSC1 and TSC2 , as negative regulators for TOR signaling .
	manualset3
123196	9	404261	13	NULL	NULL	0	NULL	One 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the recent breakthrough studies in TOR signaling resulted in the identification of the tuberous sclerosis complex gene products , TSC1 and TSC2 , as negative regulators for TOR signaling .
	manualset3
123197	1	404262	13	NULL	NULL	0	NULL	One 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the significant outcomes of this state is accelerated protein degradation and muscle wasting .
	manualset3
123198	2	404262	13	NULL	NULL	0	NULL	significant outcomes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the significant outcomes of this state is accelerated protein degradation and muscle wasting .
	manualset3
123199	3	404262	13	NULL	NULL	0	NULL	state	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the significant outcomes of this state is accelerated protein degradation and muscle wasting .
	manualset3
123200	4	404262	13	NULL	NULL	0	NULL	protein degradation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the significant outcomes of this state is accelerated protein degradation and muscle wasting .
	manualset3
123201	5	404262	13	NULL	NULL	0	NULL	muscle wasting	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the significant outcomes of this state is accelerated protein degradation and muscle wasting .
	manualset3
123202	1	404263	13	NULL	NULL	0	NULL	One 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the surprises from the early crystallographic work on MHC class II molecules was the observation that individual class II molecules existed as dimers of dimers or `` superdimers , '' as they were called .
	manualset3
123203	2	404263	13	NULL	NULL	0	NULL	surprises	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the surprises from the early crystallographic work on MHC class II molecules was the observation that individual class II molecules existed as dimers of dimers or `` superdimers , '' as they were called .
	manualset3
123204	3	404263	13	NULL	NULL	0	NULL	crystallographic work	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the surprises from the early crystallographic work on MHC class II molecules was the observation that individual class II molecules existed as dimers of dimers or `` superdimers , '' as they were called .
	manualset3
123205	4	404263	13	NULL	NULL	0	NULL	 MHC class II molecules	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the surprises from the early crystallographic work on MHC class II molecules was the observation that individual class II molecules existed as dimers of dimers or `` superdimers , '' as they were called .
	manualset3
123206	5	404263	13	NULL	NULL	0	NULL	observation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the surprises from the early crystallographic work on MHC class II molecules was the observation that individual class II molecules existed as dimers of dimers or `` superdimers , '' as they were called .
	manualset3
123207	6	404263	13	NULL	NULL	0	NULL	 individual class II molecules	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the surprises from the early crystallographic work on MHC class II molecules was the observation that individual class II molecules existed as dimers of dimers or `` superdimers , '' as they were called .
	manualset3
123208	7	404263	13	NULL	NULL	0	NULL	dimers of dimers	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the surprises from the early crystallographic work on MHC class II molecules was the observation that individual class II molecules existed as dimers of dimers or `` superdimers , '' as they were called .
	manualset3
123209	8	404263	13	NULL	NULL	0	NULL	superdimers 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the surprises from the early crystallographic work on MHC class II molecules was the observation that individual class II molecules existed as dimers of dimers or `` superdimers , '' as they were called .
	manualset3
123210	1	404264	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of them , named RIMKLA , is almost exclusively expressed in the CNS , whereas RIMKLB , which shares 65 % sequence identity with RIMKLA , is expressed in CNS and testis .
	manualset3
123211	2	404264	13	NULL	NULL	0	NULL	RIMKLA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One of them , named RIMKLA , is almost exclusively expressed in the CNS , whereas RIMKLB , which shares 65 % sequence identity with RIMKLA , is expressed in CNS and testis .
	manualset3
123212	3	404264	13	NULL	NULL	NULL	NULL	CNS	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	One of them , named RIMKLA , is almost exclusively expressed in the CNS , whereas RIMKLB , which shares 65 % sequence identity with RIMKLA , is expressed in CNS and testis .
	manualset3
123213	4	404264	13	NULL	NULL	0	NULL	RIMKLB 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One of them , named RIMKLA , is almost exclusively expressed in the CNS , whereas RIMKLB , which shares 65 % sequence identity with RIMKLA , is expressed in CNS and testis .
	manualset3
123214	5	404264	13	NULL	NULL	0	NULL	65 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One of them , named RIMKLA , is almost exclusively expressed in the CNS , whereas RIMKLB , which shares 65 % sequence identity with RIMKLA , is expressed in CNS and testis .
	manualset3
123215	6	404264	13	NULL	NULL	0	NULL	sequence identity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One of them , named RIMKLA , is almost exclusively expressed in the CNS , whereas RIMKLB , which shares 65 % sequence identity with RIMKLA , is expressed in CNS and testis .
	manualset3
123216	7	404264	13	NULL	NULL	0	NULL	RIMKLA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One of them , named RIMKLA , is almost exclusively expressed in the CNS , whereas RIMKLB , which shares 65 % sequence identity with RIMKLA , is expressed in CNS and testis .
	manualset3
123217	8	404264	13	NULL	NULL	0	NULL	CNS	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	One of them , named RIMKLA , is almost exclusively expressed in the CNS , whereas RIMKLB , which shares 65 % sequence identity with RIMKLA , is expressed in CNS and testis .
	manualset3
123218	9	404264	13	NULL	NULL	0	NULL	testis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	One of them , named RIMKLA , is almost exclusively expressed in the CNS , whereas RIMKLB , which shares 65 % sequence identity with RIMKLA , is expressed in CNS and testis .
	manualset3
123219	1	404265	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of these mapped to the baboon ortholog of human chromosome 1p32-p34 and influenced concentrations of LDL-cholesterol on Basal and high-fat , low-cholesterol diets .
	manualset3
123220	2	404265	13	NULL	NULL	0	NULL	baboon ortholog 	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	One of these mapped to the baboon ortholog of human chromosome 1p32-p34 and influenced concentrations of LDL-cholesterol on Basal and high-fat , low-cholesterol diets .
	manualset3
123221	3	404265	13	NULL	NULL	0	NULL	human chromosome 1p32-p34	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	One of these mapped to the baboon ortholog of human chromosome 1p32-p34 and influenced concentrations of LDL-cholesterol on Basal and high-fat , low-cholesterol diets .
	manualset3
123222	4	404265	13	NULL	NULL	0	NULL	concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One of these mapped to the baboon ortholog of human chromosome 1p32-p34 and influenced concentrations of LDL-cholesterol on Basal and high-fat , low-cholesterol diets .
	manualset3
123223	5	404265	13	NULL	NULL	0	NULL	LDL-cholesterol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	One of these mapped to the baboon ortholog of human chromosome 1p32-p34 and influenced concentrations of LDL-cholesterol on Basal and high-fat , low-cholesterol diets .
	manualset3
123224	6	404265	13	NULL	NULL	0	NULL	Basal diets	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	One of these mapped to the baboon ortholog of human chromosome 1p32-p34 and influenced concentrations of LDL-cholesterol on Basal and high-fat , low-cholesterol diets .
	manualset3
123225	7	404265	13	NULL	NULL	0	NULL	high-fat , low-cholesterol diets	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	One of these mapped to the baboon ortholog of human chromosome 1p32-p34 and influenced concentrations of LDL-cholesterol on Basal and high-fat , low-cholesterol diets .
	manualset3
123226	1	404266	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of these plants T1-47 , and its siblings T2-1 .2 and T2-1 .5 are the subject of the present work .
	manualset3
123227	2	404266	13	NULL	NULL	0	NULL	plants T1-47 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	One of these plants T1-47 , and its siblings T2-1 .2 and T2-1 .5 are the subject of the present work .
	manualset3
123228	3	404266	13	NULL	NULL	0	NULL	siblings	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	One of these plants T1-47 , and its siblings T2-1 .2 and T2-1 .5 are the subject of the present work .
	manualset3
123229	4	404266	13	NULL	NULL	0	NULL	T2-1 .2	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	One of these plants T1-47 , and its siblings T2-1 .2 and T2-1 .5 are the subject of the present work .
	manualset3
123230	5	404266	13	NULL	NULL	0	NULL	T2-1 .5	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	One of these plants T1-47 , and its siblings T2-1 .2 and T2-1 .5 are the subject of the present work .
	manualset3
123231	6	404266	13	NULL	NULL	0	NULL	work	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of these plants T1-47 , and its siblings T2-1 .2 and T2-1 .5 are the subject of the present work .
	manualset3
123232	1	404267	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of these roles is that it provides an effective autoregulatory mechanism which protects the host from excessive inflammation and tissue damage which is in part initiated by the Th1 driven pro-inflammatory immune responses during infections ( such as TB , HIV and malaria ) .
	manualset3
123233	2	404267	13	NULL	NULL	0	NULL	roles	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of these roles is that it provides an effective autoregulatory mechanism which protects the host from excessive inflammation and tissue damage which is in part initiated by the Th1 driven pro-inflammatory immune responses during infections ( such as TB , HIV and malaria ) .
	manualset3
123234	3	404267	13	NULL	NULL	0	NULL	autoregulatory mechanism 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One of these roles is that it provides an effective autoregulatory mechanism which protects the host from excessive inflammation and tissue damage which is in part initiated by the Th1 driven pro-inflammatory immune responses during infections ( such as TB , HIV and malaria ) .
	manualset3
123235	4	404267	13	NULL	NULL	0	NULL	host	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	One of these roles is that it provides an effective autoregulatory mechanism which protects the host from excessive inflammation and tissue damage which is in part initiated by the Th1 driven pro-inflammatory immune responses during infections ( such as TB , HIV and malaria ) .
	manualset3
123236	5	404267	13	NULL	NULL	0	NULL	excessive inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of these roles is that it provides an effective autoregulatory mechanism which protects the host from excessive inflammation and tissue damage which is in part initiated by the Th1 driven pro-inflammatory immune responses during infections ( such as TB , HIV and malaria ) .
	manualset3
123237	6	404267	13	NULL	NULL	0	NULL	tissue damage 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of these roles is that it provides an effective autoregulatory mechanism which protects the host from excessive inflammation and tissue damage which is in part initiated by the Th1 driven pro-inflammatory immune responses during infections ( such as TB , HIV and malaria ) .
	manualset3
123238	7	404267	13	NULL	NULL	0	NULL	Th1 driven pro-inflammatory immune responses 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of these roles is that it provides an effective autoregulatory mechanism which protects the host from excessive inflammation and tissue damage which is in part initiated by the Th1 driven pro-inflammatory immune responses during infections ( such as TB , HIV and malaria ) .
	manualset3
123239	8	404267	13	NULL	NULL	0	NULL	infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of these roles is that it provides an effective autoregulatory mechanism which protects the host from excessive inflammation and tissue damage which is in part initiated by the Th1 driven pro-inflammatory immune responses during infections ( such as TB , HIV and malaria ) .
	manualset3
123240	9	404267	13	NULL	NULL	0	NULL	TB	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of these roles is that it provides an effective autoregulatory mechanism which protects the host from excessive inflammation and tissue damage which is in part initiated by the Th1 driven pro-inflammatory immune responses during infections ( such as TB , HIV and malaria ) .
	manualset3
123241	10	404267	13	NULL	NULL	0	NULL	HIV	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of these roles is that it provides an effective autoregulatory mechanism which protects the host from excessive inflammation and tissue damage which is in part initiated by the Th1 driven pro-inflammatory immune responses during infections ( such as TB , HIV and malaria ) .
	manualset3
123242	11	404267	13	NULL	NULL	0	NULL	malaria	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of these roles is that it provides an effective autoregulatory mechanism which protects the host from excessive inflammation and tissue damage which is in part initiated by the Th1 driven pro-inflammatory immune responses during infections ( such as TB , HIV and malaria ) .
	manualset3
123243	1	404268	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One open reading frame encodes a protein with 942 amino acids showing 38 % identity with DNA polymerase I from E. coli .
	manualset3
123244	2	404268	13	NULL	NULL	0	NULL	open reading frame 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	One open reading frame encodes a protein with 942 amino acids showing 38 % identity with DNA polymerase I from E. coli .
	manualset3
123245	3	404268	13	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One open reading frame encodes a protein with 942 amino acids showing 38 % identity with DNA polymerase I from E. coli .
	manualset3
123246	4	404268	13	NULL	NULL	0	NULL	942 amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	One open reading frame encodes a protein with 942 amino acids showing 38 % identity with DNA polymerase I from E. coli .
	manualset3
123247	5	404268	13	NULL	NULL	0	NULL	38 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One open reading frame encodes a protein with 942 amino acids showing 38 % identity with DNA polymerase I from E. coli .
	manualset3
123248	6	404268	13	NULL	NULL	0	NULL	identity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One open reading frame encodes a protein with 942 amino acids showing 38 % identity with DNA polymerase I from E. coli .
	manualset3
123249	7	404268	13	NULL	NULL	0	NULL	DNA polymerase I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One open reading frame encodes a protein with 942 amino acids showing 38 % identity with DNA polymerase I from E. coli .
	manualset3
123250	8	404268	13	NULL	NULL	0	NULL	E. coli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	One open reading frame encodes a protein with 942 amino acids showing 38 % identity with DNA polymerase I from E. coli .
	manualset3
123251	1	404269	13	NULL	NULL	0	NULL	dihydroampicillin ( 3 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A dihydroampicillin ( 3 ) and a dihydrocephalexin ( 4 ) have been synthesized by condensing alpha - ( cyclohexa-1 , 3-dienyl ) glycyl chloride with 6-aminopenicillanic acid ( 1 ) and 7-deacetoxycephalosporanic acid ( 2 ) respectively .
	manualset3
123252	2	404269	13	NULL	NULL	0	NULL	dihydrocephalexin ( 4 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A dihydroampicillin ( 3 ) and a dihydrocephalexin ( 4 ) have been synthesized by condensing alpha - ( cyclohexa-1 , 3-dienyl ) glycyl chloride with 6-aminopenicillanic acid ( 1 ) and 7-deacetoxycephalosporanic acid ( 2 ) respectively .
	manualset3
123254	3	404269	13	NULL	NULL	0	NULL	condensing 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A dihydroampicillin ( 3 ) and a dihydrocephalexin ( 4 ) have been synthesized by condensing alpha - ( cyclohexa-1 , 3-dienyl ) glycyl chloride with 6-aminopenicillanic acid ( 1 ) and 7-deacetoxycephalosporanic acid ( 2 ) respectively .
	manualset3
123255	4	404269	13	NULL	NULL	0	NULL	alpha - ( cyclohexa-1 , 3-dienyl ) glycyl chloride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A dihydroampicillin ( 3 ) and a dihydrocephalexin ( 4 ) have been synthesized by condensing alpha - ( cyclohexa-1 , 3-dienyl ) glycyl chloride with 6-aminopenicillanic acid ( 1 ) and 7-deacetoxycephalosporanic acid ( 2 ) respectively .
	manualset3
123256	5	404269	13	NULL	NULL	0	NULL	6-aminopenicillanic acid ( 1 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A dihydroampicillin ( 3 ) and a dihydrocephalexin ( 4 ) have been synthesized by condensing alpha - ( cyclohexa-1 , 3-dienyl ) glycyl chloride with 6-aminopenicillanic acid ( 1 ) and 7-deacetoxycephalosporanic acid ( 2 ) respectively .
	manualset3
123257	6	404269	13	NULL	NULL	0	NULL	7-deacetoxycephalosporanic acid ( 2 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A dihydroampicillin ( 3 ) and a dihydrocephalexin ( 4 ) have been synthesized by condensing alpha - ( cyclohexa-1 , 3-dienyl ) glycyl chloride with 6-aminopenicillanic acid ( 1 ) and 7-deacetoxycephalosporanic acid ( 2 ) respectively .
	manualset3
123258	1	404270	13	NULL	NULL	0	NULL	One pair	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One pair of unique enantiomorphic alkaloidal glycosides T-1 and T-2 was isolated and their structures were elucidated unambiguously by HR-MS , CD , 1D and 2D NMR spectrum .
	manualset3
123259	2	404270	13	NULL	NULL	0	NULL	enantiomorphic alkaloidal glycosides T-1 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	One pair of unique enantiomorphic alkaloidal glycosides T-1 and T-2 was isolated and their structures were elucidated unambiguously by HR-MS , CD , 1D and 2D NMR spectrum .
	manualset3
123260	3	404270	13	NULL	NULL	0	NULL	enantiomorphic alkaloidal glycosides T-2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	One pair of unique enantiomorphic alkaloidal glycosides T-1 and T-2 was isolated and their structures were elucidated unambiguously by HR-MS , CD , 1D and 2D NMR spectrum .
	manualset3
123261	4	404270	13	NULL	NULL	0	NULL	structures	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One pair of unique enantiomorphic alkaloidal glycosides T-1 and T-2 was isolated and their structures were elucidated unambiguously by HR-MS , CD , 1D and 2D NMR spectrum .
	manualset3
123262	5	404270	13	NULL	NULL	0	NULL	HR-MS	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	One pair of unique enantiomorphic alkaloidal glycosides T-1 and T-2 was isolated and their structures were elucidated unambiguously by HR-MS , CD , 1D and 2D NMR spectrum .
	manualset3
123263	6	404270	13	NULL	NULL	0	NULL	CD	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	One pair of unique enantiomorphic alkaloidal glycosides T-1 and T-2 was isolated and their structures were elucidated unambiguously by HR-MS , CD , 1D and 2D NMR spectrum .
	manualset3
123264	7	404270	13	NULL	NULL	0	NULL	1D NMR spectrum	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	One pair of unique enantiomorphic alkaloidal glycosides T-1 and T-2 was isolated and their structures were elucidated unambiguously by HR-MS , CD , 1D and 2D NMR spectrum .
	manualset3
123265	8	404270	13	NULL	NULL	0	NULL	2D NMR spectrum	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	One pair of unique enantiomorphic alkaloidal glycosides T-1 and T-2 was isolated and their structures were elucidated unambiguously by HR-MS , CD , 1D and 2D NMR spectrum .
	manualset3
123266	1	404271	13	NULL	NULL	0	NULL	One patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient , in the insulin lispro treatment arm , discontinued because early interruption criteria were met after 7 hours .
	manualset3
123267	2	404271	13	NULL	NULL	0	NULL	insulin lispro	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient , in the insulin lispro treatment arm , discontinued because early interruption criteria were met after 7 hours .
	manualset3
123268	3	404271	13	NULL	NULL	0	NULL	treatment arm	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient , in the insulin lispro treatment arm , discontinued because early interruption criteria were met after 7 hours .
	manualset3
123269	4	404271	13	NULL	NULL	0	NULL	interruption criteria	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient , in the insulin lispro treatment arm , discontinued because early interruption criteria were met after 7 hours .
	manualset3
123270	5	404271	13	NULL	NULL	0	NULL	after 7 hours	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient , in the insulin lispro treatment arm , discontinued because early interruption criteria were met after 7 hours .
	manualset3
123271	1	404272	13	NULL	NULL	0	NULL	One patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient died 18 months after her procedure , possibly owing to aneurysm expansion .
	manualset3
123272	2	404272	13	NULL	NULL	0	NULL	18 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient died 18 months after her procedure , possibly owing to aneurysm expansion .
	manualset3
123273	3	404272	13	NULL	NULL	0	NULL	procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient died 18 months after her procedure , possibly owing to aneurysm expansion .
	manualset3
123274	4	404272	13	NULL	NULL	0	NULL	aneurysm expansion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient died 18 months after her procedure , possibly owing to aneurysm expansion .
	manualset3
123275	1	404273	13	NULL	NULL	0	NULL	One patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient died with rapidly progressive disease but the other has had an excellent response to therapy with high-dose melphalan ( HDM , 200 mg/m2 ) and peripheral blood stem cell rescue .
	manualset3
123276	2	404273	13	NULL	NULL	0	NULL	progressive disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient died with rapidly progressive disease but the other has had an excellent response to therapy with high-dose melphalan ( HDM , 200 mg/m2 ) and peripheral blood stem cell rescue .
	manualset3
123277	3	404273	13	NULL	NULL	0	NULL	excellent response 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient died with rapidly progressive disease but the other has had an excellent response to therapy with high-dose melphalan ( HDM , 200 mg/m2 ) and peripheral blood stem cell rescue .
	manualset3
123278	4	404273	13	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient died with rapidly progressive disease but the other has had an excellent response to therapy with high-dose melphalan ( HDM , 200 mg/m2 ) and peripheral blood stem cell rescue .
	manualset3
123279	5	404273	13	NULL	NULL	0	NULL	high-dose melphalan	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient died with rapidly progressive disease but the other has had an excellent response to therapy with high-dose melphalan ( HDM , 200 mg/m2 ) and peripheral blood stem cell rescue .
	manualset3
123280	6	404273	13	NULL	NULL	0	NULL	HDM , 200 mg/m2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient died with rapidly progressive disease but the other has had an excellent response to therapy with high-dose melphalan ( HDM , 200 mg/m2 ) and peripheral blood stem cell rescue .
	manualset3
123281	7	404273	13	NULL	NULL	0	NULL	peripheral blood stem cell 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient died with rapidly progressive disease but the other has had an excellent response to therapy with high-dose melphalan ( HDM , 200 mg/m2 ) and peripheral blood stem cell rescue .
	manualset3
123282	8	404273	13	NULL	NULL	0	NULL	rescue	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient died with rapidly progressive disease but the other has had an excellent response to therapy with high-dose melphalan ( HDM , 200 mg/m2 ) and peripheral blood stem cell rescue .
	manualset3
123283	1	404274	13	NULL	NULL	0	NULL	One patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient had no p53 mutation in his leukemic cells during chronic phase of ATL , but had a homozygous point mutation at codon 273 ( Arg to His ) when he progressed to acute ATL .
	manualset3
123284	2	404274	13	NULL	NULL	0	NULL	p53 mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient had no p53 mutation in his leukemic cells during chronic phase of ATL , but had a homozygous point mutation at codon 273 ( Arg to His ) when he progressed to acute ATL .
	manualset3
123285	3	404274	13	NULL	NULL	0	NULL	leukemic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient had no p53 mutation in his leukemic cells during chronic phase of ATL , but had a homozygous point mutation at codon 273 ( Arg to His ) when he progressed to acute ATL .
	manualset3
123286	4	404274	13	NULL	NULL	0	NULL	chronic phase of ATL	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient had no p53 mutation in his leukemic cells during chronic phase of ATL , but had a homozygous point mutation at codon 273 ( Arg to His ) when he progressed to acute ATL .
	manualset3
123287	5	404274	13	NULL	NULL	0	NULL	homozygous point mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient had no p53 mutation in his leukemic cells during chronic phase of ATL , but had a homozygous point mutation at codon 273 ( Arg to His ) when he progressed to acute ATL .
	manualset3
123288	6	404274	13	NULL	NULL	NULL	NULL	codon 273	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	One patient had no p53 mutation in his leukemic cells during chronic phase of ATL , but had a homozygous point mutation at codon 273 ( Arg to His ) when he progressed to acute ATL .
	manualset3
123289	7	404274	13	NULL	NULL	0	NULL	Arg	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient had no p53 mutation in his leukemic cells during chronic phase of ATL , but had a homozygous point mutation at codon 273 ( Arg to His ) when he progressed to acute ATL .
	manualset3
123290	8	404274	13	NULL	NULL	0	NULL	His	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient had no p53 mutation in his leukemic cells during chronic phase of ATL , but had a homozygous point mutation at codon 273 ( Arg to His ) when he progressed to acute ATL .
	manualset3
123291	9	404274	13	NULL	NULL	0	NULL	acute ATL	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient had no p53 mutation in his leukemic cells during chronic phase of ATL , but had a homozygous point mutation at codon 273 ( Arg to His ) when he progressed to acute ATL .
	manualset3
123292	1	404275	13	NULL	NULL	0	NULL	One patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient who refused operation continued to have recurrent pancreatitis 41 months after diagnosis .
	manualset3
123293	2	404275	13	NULL	NULL	0	NULL	operation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient who refused operation continued to have recurrent pancreatitis 41 months after diagnosis .
	manualset3
123294	3	404275	13	NULL	NULL	0	NULL	recurrent pancreatitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient who refused operation continued to have recurrent pancreatitis 41 months after diagnosis .
	manualset3
123295	4	404275	13	NULL	NULL	0	NULL	41 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient who refused operation continued to have recurrent pancreatitis 41 months after diagnosis .
	manualset3
123296	5	404275	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient who refused operation continued to have recurrent pancreatitis 41 months after diagnosis .
	manualset3
123297	1	404276	13	NULL	NULL	0	NULL	One patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient who was still PCR positive 27 months after BMT became negative 12 months later .
	manualset3
123298	2	404276	13	NULL	NULL	0	NULL	PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient who was still PCR positive 27 months after BMT became negative 12 months later .
	manualset3
123299	3	404276	13	NULL	NULL	0	NULL	27 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient who was still PCR positive 27 months after BMT became negative 12 months later .
	manualset3
123300	4	404276	13	NULL	NULL	0	NULL	BMT 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient who was still PCR positive 27 months after BMT became negative 12 months later .
	manualset3
123301	5	404276	13	NULL	NULL	0	NULL	12 months 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	One patient who was still PCR positive 27 months after BMT became negative 12 months later .
	manualset3
123302	1	404277	13	NULL	NULL	0	NULL	dimeric Rep protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A dimeric Rep protein initiates replication of a linear archaeal virus genome : implications for the Rep mechanism and viral replication .
	manualset3
123304	3	404277	13	NULL	NULL	0	NULL	replication 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A dimeric Rep protein initiates replication of a linear archaeal virus genome : implications for the Rep mechanism and viral replication .
	manualset3
123305	4	404277	13	NULL	NULL	0	NULL	linear archaeal virus genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A dimeric Rep protein initiates replication of a linear archaeal virus genome : implications for the Rep mechanism and viral replication .
	manualset3
123306	5	404277	13	NULL	NULL	0	NULL	implications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A dimeric Rep protein initiates replication of a linear archaeal virus genome : implications for the Rep mechanism and viral replication .
	manualset3
123307	6	404277	13	NULL	NULL	0	NULL	Rep mechanism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A dimeric Rep protein initiates replication of a linear archaeal virus genome : implications for the Rep mechanism and viral replication .
	manualset3
123308	7	404277	13	NULL	NULL	0	NULL	viral replication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A dimeric Rep protein initiates replication of a linear archaeal virus genome : implications for the Rep mechanism and viral replication .
	manualset3
123309	1	404278	13	NULL	NULL	0	NULL	One platform	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	One platform , multiple insights .
	manualset3
123310	2	404278	13	NULL	NULL	NULL	NULL	multiple insights	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	One platform , multiple insights .
	manualset3
123311	1	404279	13	NULL	NULL	0	NULL	One reason 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One reason for the influence of PEG is that ACP with different PEG content could have two types of unit structures that tend to form alpha-TCP and beta-TCP after crystallization .
	manualset3
123312	2	404279	13	NULL	NULL	0	NULL	influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One reason for the influence of PEG is that ACP with different PEG content could have two types of unit structures that tend to form alpha-TCP and beta-TCP after crystallization .
	manualset3
123313	3	404279	13	NULL	NULL	0	NULL	PEG	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	One reason for the influence of PEG is that ACP with different PEG content could have two types of unit structures that tend to form alpha-TCP and beta-TCP after crystallization .
	manualset3
123314	4	404279	13	NULL	NULL	0	NULL	ACP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	One reason for the influence of PEG is that ACP with different PEG content could have two types of unit structures that tend to form alpha-TCP and beta-TCP after crystallization .
	manualset3
123315	5	404279	13	NULL	NULL	0	NULL	PEG content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One reason for the influence of PEG is that ACP with different PEG content could have two types of unit structures that tend to form alpha-TCP and beta-TCP after crystallization .
	manualset3
123316	6	404279	13	NULL	NULL	0	NULL	two types	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One reason for the influence of PEG is that ACP with different PEG content could have two types of unit structures that tend to form alpha-TCP and beta-TCP after crystallization .
	manualset3
123317	7	404279	13	NULL	NULL	0	NULL	unit structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	One reason for the influence of PEG is that ACP with different PEG content could have two types of unit structures that tend to form alpha-TCP and beta-TCP after crystallization .
	manualset3
123318	8	404279	13	NULL	NULL	0	NULL	alpha-TCP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One reason for the influence of PEG is that ACP with different PEG content could have two types of unit structures that tend to form alpha-TCP and beta-TCP after crystallization .
	manualset3
123319	9	404279	13	NULL	NULL	0	NULL	beta-TCP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One reason for the influence of PEG is that ACP with different PEG content could have two types of unit structures that tend to form alpha-TCP and beta-TCP after crystallization .
	manualset3
123320	10	404279	13	NULL	NULL	0	NULL	crystallization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One reason for the influence of PEG is that ACP with different PEG content could have two types of unit structures that tend to form alpha-TCP and beta-TCP after crystallization .
	manualset3
123321	1	404280	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One selected miniprotein-derived thrombopoietin agonist was almost as active as natural thrombopoietin with regard to stimulation of megakaryocyte colony formation from human bone marrow mononuclear cells , and elicited doubling of platelet counts in mice .
	manualset3
123322	2	404280	13	NULL	NULL	0	NULL	miniprotein-derived thrombopoietin agonist	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	One selected miniprotein-derived thrombopoietin agonist was almost as active as natural thrombopoietin with regard to stimulation of megakaryocyte colony formation from human bone marrow mononuclear cells , and elicited doubling of platelet counts in mice .
	manualset3
123323	3	404280	13	NULL	NULL	0	NULL	thrombopoietin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One selected miniprotein-derived thrombopoietin agonist was almost as active as natural thrombopoietin with regard to stimulation of megakaryocyte colony formation from human bone marrow mononuclear cells , and elicited doubling of platelet counts in mice .
	manualset3
123324	4	404280	13	NULL	NULL	0	NULL	stimulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One selected miniprotein-derived thrombopoietin agonist was almost as active as natural thrombopoietin with regard to stimulation of megakaryocyte colony formation from human bone marrow mononuclear cells , and elicited doubling of platelet counts in mice .
	manualset3
123325	5	404280	13	NULL	NULL	0	NULL	megakaryocyte colony formation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One selected miniprotein-derived thrombopoietin agonist was almost as active as natural thrombopoietin with regard to stimulation of megakaryocyte colony formation from human bone marrow mononuclear cells , and elicited doubling of platelet counts in mice .
	manualset3
123326	6	404280	13	NULL	NULL	0	NULL	human bone marrow mononuclear cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	One selected miniprotein-derived thrombopoietin agonist was almost as active as natural thrombopoietin with regard to stimulation of megakaryocyte colony formation from human bone marrow mononuclear cells , and elicited doubling of platelet counts in mice .
	manualset3
123327	7	404280	13	NULL	NULL	0	NULL	platelet counts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One selected miniprotein-derived thrombopoietin agonist was almost as active as natural thrombopoietin with regard to stimulation of megakaryocyte colony formation from human bone marrow mononuclear cells , and elicited doubling of platelet counts in mice .
	manualset3
123328	8	404280	13	NULL	NULL	0	NULL	mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	One selected miniprotein-derived thrombopoietin agonist was almost as active as natural thrombopoietin with regard to stimulation of megakaryocyte colony formation from human bone marrow mononuclear cells , and elicited doubling of platelet counts in mice .
	manualset3
123329	1	404281	13	NULL	NULL	0	NULL	One side effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One side effect is hypotension , usually ascribed to a depression of cardiac contractility , while their effects on the resistance vessels are more controversial : both vasodilation and vasoconstriction have been described .
	manualset3
123330	2	404281	13	NULL	NULL	0	NULL	hypotension 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One side effect is hypotension , usually ascribed to a depression of cardiac contractility , while their effects on the resistance vessels are more controversial : both vasodilation and vasoconstriction have been described .
	manualset3
123331	3	404281	13	NULL	NULL	0	NULL	depression of cardiac contractility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One side effect is hypotension , usually ascribed to a depression of cardiac contractility , while their effects on the resistance vessels are more controversial : both vasodilation and vasoconstriction have been described .
	manualset3
123332	4	404281	13	NULL	NULL	0	NULL	effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One side effect is hypotension , usually ascribed to a depression of cardiac contractility , while their effects on the resistance vessels are more controversial : both vasodilation and vasoconstriction have been described .
	manualset3
123333	5	404281	13	NULL	NULL	0	NULL	resistance vessels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	One side effect is hypotension , usually ascribed to a depression of cardiac contractility , while their effects on the resistance vessels are more controversial : both vasodilation and vasoconstriction have been described .
	manualset3
123334	6	404281	13	NULL	NULL	0	NULL	vasodilation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One side effect is hypotension , usually ascribed to a depression of cardiac contractility , while their effects on the resistance vessels are more controversial : both vasodilation and vasoconstriction have been described .
	manualset3
123335	7	404281	13	NULL	NULL	0	NULL	vasoconstriction 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One side effect is hypotension , usually ascribed to a depression of cardiac contractility , while their effects on the resistance vessels are more controversial : both vasodilation and vasoconstriction have been described .
	manualset3
123336	1	404282	13	NULL	NULL	0	NULL	Body measurements	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( Body measurements and morphological signs of maturity in newborn infants after hyperemesis gravidarum ) .
	manualset3
123337	2	404282	13	NULL	NULL	0	NULL	morphological signs 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Body measurements and morphological signs of maturity in newborn infants after hyperemesis gravidarum ) .
	manualset3
123338	3	404282	13	NULL	NULL	0	NULL	maturity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Body measurements and morphological signs of maturity in newborn infants after hyperemesis gravidarum ) .
	manualset3
123339	4	404282	13	NULL	NULL	0	NULL	newborn infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Body measurements and morphological signs of maturity in newborn infants after hyperemesis gravidarum ) .
	manualset3
123340	5	404282	13	NULL	NULL	0	NULL	hyperemesis gravidarum	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Body measurements and morphological signs of maturity in newborn infants after hyperemesis gravidarum ) .
	manualset3
123341	1	404283	13	NULL	NULL	NULL	NULL	dinitrobenzene derivative of neomycin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A dinitrobenzene derivative of neomycin is formed and then chromatographed isocratically on a normal-phase system .
	manualset3
123342	2	404283	13	NULL	NULL	0	NULL	normal-phase system	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A dinitrobenzene derivative of neomycin is formed and then chromatographed isocratically on a normal-phase system .
	manualset3
123343	1	404284	13	NULL	NULL	0	NULL	One step	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One step in this `` side-path '' electron conduction is thought to be mediated by Car oxidation .
	manualset3
123344	2	404284	13	NULL	NULL	0	NULL	electron conduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One step in this `` side-path '' electron conduction is thought to be mediated by Car oxidation .
	manualset3
123345	3	404284	13	NULL	NULL	0	NULL	Car oxidation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One step in this `` side-path '' electron conduction is thought to be mediated by Car oxidation .
	manualset3
123346	1	404285	13	NULL	NULL	0	NULL	One subpopulation 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	One subpopulation comprised of a few hundreds of neurons projects to the pacemaker nucleus in the medulla oblongata , thus constituting the prepacemaker nucleus portion of this complex .
	manualset3
123347	2	404285	13	NULL	NULL	0	NULL	few hundreds	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One subpopulation comprised of a few hundreds of neurons projects to the pacemaker nucleus in the medulla oblongata , thus constituting the prepacemaker nucleus portion of this complex .
	manualset3
123348	3	404285	13	NULL	NULL	0	NULL	neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	One subpopulation comprised of a few hundreds of neurons projects to the pacemaker nucleus in the medulla oblongata , thus constituting the prepacemaker nucleus portion of this complex .
	manualset3
123349	4	404285	13	NULL	NULL	0	NULL	projects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One subpopulation comprised of a few hundreds of neurons projects to the pacemaker nucleus in the medulla oblongata , thus constituting the prepacemaker nucleus portion of this complex .
	manualset3
123350	5	404285	13	NULL	NULL	0	NULL	pacemaker nucleus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	One subpopulation comprised of a few hundreds of neurons projects to the pacemaker nucleus in the medulla oblongata , thus constituting the prepacemaker nucleus portion of this complex .
	manualset3
123351	6	404285	13	NULL	NULL	0	NULL	medulla oblongata	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	One subpopulation comprised of a few hundreds of neurons projects to the pacemaker nucleus in the medulla oblongata , thus constituting the prepacemaker nucleus portion of this complex .
	manualset3
123352	7	404285	13	NULL	NULL	0	NULL	prepacemaker nucleus portion 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	One subpopulation comprised of a few hundreds of neurons projects to the pacemaker nucleus in the medulla oblongata , thus constituting the prepacemaker nucleus portion of this complex .
	manualset3
123353	8	404285	13	NULL	NULL	0	NULL	complex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	One subpopulation comprised of a few hundreds of neurons projects to the pacemaker nucleus in the medulla oblongata , thus constituting the prepacemaker nucleus portion of this complex .
	manualset3
123354	1	404286	13	NULL	NULL	0	NULL	One subpopulation	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	One subpopulation of effector/memory Foxp3 ( + ) T cells develops in the thymic medulla , whereas the second is thymic independent .
	manualset3
123355	2	404286	13	NULL	NULL	0	NULL	effector/memory Foxp3 ( + ) T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	One subpopulation of effector/memory Foxp3 ( + ) T cells develops in the thymic medulla , whereas the second is thymic independent .
	manualset3
123356	3	404286	13	NULL	NULL	0	NULL	thymic medulla	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	One subpopulation of effector/memory Foxp3 ( + ) T cells develops in the thymic medulla , whereas the second is thymic independent .
	manualset3
123357	1	404287	13	NULL	NULL	0	NULL	One testis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	One testis and epididymis were removed and weighed .
	manualset3
123358	2	404287	13	NULL	NULL	0	NULL	epididymis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	One testis and epididymis were removed and weighed .
	manualset3
123359	1	404288	13	NULL	NULL	NULL	NULL	One	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	One yielding seat had k = 20 kN/m and j = 1.4 degrees / kN simulating a high-retention seat ( 1997 Grand Prix ) and another k = 20 kN/m and j = 3.4 degrees / kN simulating a 1980s to 1990s yielding seat ( 1990 Buick Park Avenue ) .
	manualset3
123360	2	404288	13	NULL	NULL	0	NULL	k = 20 kN/m 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One yielding seat had k = 20 kN/m and j = 1.4 degrees / kN simulating a high-retention seat ( 1997 Grand Prix ) and another k = 20 kN/m and j = 3.4 degrees / kN simulating a 1980s to 1990s yielding seat ( 1990 Buick Park Avenue ) .
	manualset3
123361	3	404288	13	NULL	NULL	0	NULL	j = 1.4 degrees / kN	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One yielding seat had k = 20 kN/m and j = 1.4 degrees / kN simulating a high-retention seat ( 1997 Grand Prix ) and another k = 20 kN/m and j = 3.4 degrees / kN simulating a 1980s to 1990s yielding seat ( 1990 Buick Park Avenue ) .
	manualset3
123362	4	404288	13	NULL	NULL	0	NULL	high-retention seat	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	One yielding seat had k = 20 kN/m and j = 1.4 degrees / kN simulating a high-retention seat ( 1997 Grand Prix ) and another k = 20 kN/m and j = 3.4 degrees / kN simulating a 1980s to 1990s yielding seat ( 1990 Buick Park Avenue ) .
	manualset3
123363	5	404288	13	NULL	NULL	0	NULL	1997	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	One yielding seat had k = 20 kN/m and j = 1.4 degrees / kN simulating a high-retention seat ( 1997 Grand Prix ) and another k = 20 kN/m and j = 3.4 degrees / kN simulating a 1980s to 1990s yielding seat ( 1990 Buick Park Avenue ) .
	manualset3
123364	6	404288	13	NULL	NULL	0	NULL	Grand Prix	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One yielding seat had k = 20 kN/m and j = 1.4 degrees / kN simulating a high-retention seat ( 1997 Grand Prix ) and another k = 20 kN/m and j = 3.4 degrees / kN simulating a 1980s to 1990s yielding seat ( 1990 Buick Park Avenue ) .
	manualset3
123365	7	404288	13	NULL	NULL	0	NULL	k = 20 kN/m	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One yielding seat had k = 20 kN/m and j = 1.4 degrees / kN simulating a high-retention seat ( 1997 Grand Prix ) and another k = 20 kN/m and j = 3.4 degrees / kN simulating a 1980s to 1990s yielding seat ( 1990 Buick Park Avenue ) .
	manualset3
123366	8	404288	13	NULL	NULL	0	NULL	j = 3.4 degrees / kN 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	One yielding seat had k = 20 kN/m and j = 1.4 degrees / kN simulating a high-retention seat ( 1997 Grand Prix ) and another k = 20 kN/m and j = 3.4 degrees / kN simulating a 1980s to 1990s yielding seat ( 1990 Buick Park Avenue ) .
	manualset3
123367	9	404288	13	NULL	NULL	0	NULL	1980s	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	One yielding seat had k = 20 kN/m and j = 1.4 degrees / kN simulating a high-retention seat ( 1997 Grand Prix ) and another k = 20 kN/m and j = 3.4 degrees / kN simulating a 1980s to 1990s yielding seat ( 1990 Buick Park Avenue ) .
	manualset3
123368	10	404288	13	NULL	NULL	0	NULL	1990s 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	One yielding seat had k = 20 kN/m and j = 1.4 degrees / kN simulating a high-retention seat ( 1997 Grand Prix ) and another k = 20 kN/m and j = 3.4 degrees / kN simulating a 1980s to 1990s yielding seat ( 1990 Buick Park Avenue ) .
	manualset3
123369	11	404288	13	NULL	NULL	NULL	NULL	seat	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	One yielding seat had k = 20 kN/m and j = 1.4 degrees / kN simulating a high-retention seat ( 1997 Grand Prix ) and another k = 20 kN/m and j = 3.4 degrees / kN simulating a 1980s to 1990s yielding seat ( 1990 Buick Park Avenue ) .
	manualset3
123370	12	404288	13	NULL	NULL	0	NULL	1990	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	One yielding seat had k = 20 kN/m and j = 1.4 degrees / kN simulating a high-retention seat ( 1997 Grand Prix ) and another k = 20 kN/m and j = 3.4 degrees / kN simulating a 1980s to 1990s yielding seat ( 1990 Buick Park Avenue ) .
	manualset3
123371	13	404288	13	NULL	NULL	0	NULL	Buick Park Avenue	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	One yielding seat had k = 20 kN/m and j = 1.4 degrees / kN simulating a high-retention seat ( 1997 Grand Prix ) and another k = 20 kN/m and j = 3.4 degrees / kN simulating a 1980s to 1990s yielding seat ( 1990 Buick Park Avenue ) .
	manualset3
123372	14	404288	13	NULL	NULL	NULL	NULL	seat	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	One yielding seat had k = 20 kN/m and j = 1.4 degrees / kN simulating a high-retention seat ( 1997 Grand Prix ) and another k = 20 kN/m and j = 3.4 degrees / kN simulating a 1980s to 1990s yielding seat ( 1990 Buick Park Avenue ) .
	manualset3
123373	1	404289	13	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One can of course tell the story of psychiatry based purely on medicine history , but if one examines it from the point of view of evolution , one discovers a profound meaning in its development .
	manualset3
123374	2	404289	13	NULL	NULL	0	NULL	course	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One can of course tell the story of psychiatry based purely on medicine history , but if one examines it from the point of view of evolution , one discovers a profound meaning in its development .
	manualset3
123375	3	404289	13	NULL	NULL	0	NULL	psychiatry 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	One can of course tell the story of psychiatry based purely on medicine history , but if one examines it from the point of view of evolution , one discovers a profound meaning in its development .
	manualset3
123376	4	404289	13	NULL	NULL	0	NULL	medicine history 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One can of course tell the story of psychiatry based purely on medicine history , but if one examines it from the point of view of evolution , one discovers a profound meaning in its development .
	manualset3
123377	5	404289	13	NULL	NULL	0	NULL	point of view	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One can of course tell the story of psychiatry based purely on medicine history , but if one examines it from the point of view of evolution , one discovers a profound meaning in its development .
	manualset3
123378	6	404289	13	NULL	NULL	0	NULL	evolution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One can of course tell the story of psychiatry based purely on medicine history , but if one examines it from the point of view of evolution , one discovers a profound meaning in its development .
	manualset3
123379	7	404289	13	NULL	NULL	0	NULL	meaning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One can of course tell the story of psychiatry based purely on medicine history , but if one examines it from the point of view of evolution , one discovers a profound meaning in its development .
	manualset3
123380	8	404289	13	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One can of course tell the story of psychiatry based purely on medicine history , but if one examines it from the point of view of evolution , one discovers a profound meaning in its development .
	manualset3
123381	1	404290	13	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A direct comparison of the molecular mass of the Mu-IFN-gamma receptor on intact cells versus detergent-solubilized membranes was performed using a radiolabeled photoactivated crosslinking reagent and direct hybridization with 125I-labeled IFN-gamma on Western blots of solubilized receptor .
	manualset3
123382	2	404290	13	NULL	NULL	0	NULL	molecular mass 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A direct comparison of the molecular mass of the Mu-IFN-gamma receptor on intact cells versus detergent-solubilized membranes was performed using a radiolabeled photoactivated crosslinking reagent and direct hybridization with 125I-labeled IFN-gamma on Western blots of solubilized receptor .
	manualset3
123383	3	404290	13	NULL	NULL	0	NULL	 Mu-IFN-gamma receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A direct comparison of the molecular mass of the Mu-IFN-gamma receptor on intact cells versus detergent-solubilized membranes was performed using a radiolabeled photoactivated crosslinking reagent and direct hybridization with 125I-labeled IFN-gamma on Western blots of solubilized receptor .
	manualset3
123384	4	404290	13	NULL	NULL	0	NULL	intact cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A direct comparison of the molecular mass of the Mu-IFN-gamma receptor on intact cells versus detergent-solubilized membranes was performed using a radiolabeled photoactivated crosslinking reagent and direct hybridization with 125I-labeled IFN-gamma on Western blots of solubilized receptor .
	manualset3
123385	5	404290	13	NULL	NULL	0	NULL	detergent-solubilized membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A direct comparison of the molecular mass of the Mu-IFN-gamma receptor on intact cells versus detergent-solubilized membranes was performed using a radiolabeled photoactivated crosslinking reagent and direct hybridization with 125I-labeled IFN-gamma on Western blots of solubilized receptor .
	manualset3
123386	6	404290	13	NULL	NULL	0	NULL	crosslinking reagent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A direct comparison of the molecular mass of the Mu-IFN-gamma receptor on intact cells versus detergent-solubilized membranes was performed using a radiolabeled photoactivated crosslinking reagent and direct hybridization with 125I-labeled IFN-gamma on Western blots of solubilized receptor .
	manualset3
123387	7	404290	13	NULL	NULL	NULL	NULL	hybridization 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A direct comparison of the molecular mass of the Mu-IFN-gamma receptor on intact cells versus detergent-solubilized membranes was performed using a radiolabeled photoactivated crosslinking reagent and direct hybridization with 125I-labeled IFN-gamma on Western blots of solubilized receptor .
	manualset3
123388	8	404290	13	NULL	NULL	0	NULL	125I-labeled IFN-gamma	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A direct comparison of the molecular mass of the Mu-IFN-gamma receptor on intact cells versus detergent-solubilized membranes was performed using a radiolabeled photoactivated crosslinking reagent and direct hybridization with 125I-labeled IFN-gamma on Western blots of solubilized receptor .
	manualset3
123389	9	404290	13	NULL	NULL	0	NULL	Western blots	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A direct comparison of the molecular mass of the Mu-IFN-gamma receptor on intact cells versus detergent-solubilized membranes was performed using a radiolabeled photoactivated crosslinking reagent and direct hybridization with 125I-labeled IFN-gamma on Western blots of solubilized receptor .
	manualset3
123390	10	404290	13	NULL	NULL	0	NULL	solubilized receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A direct comparison of the molecular mass of the Mu-IFN-gamma receptor on intact cells versus detergent-solubilized membranes was performed using a radiolabeled photoactivated crosslinking reagent and direct hybridization with 125I-labeled IFN-gamma on Western blots of solubilized receptor .
	manualset3
123391	1	404291	13	NULL	NULL	0	NULL	monitoring	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ongoing monitoring is essential for patients taking medicine for active tuberculosis .
	manualset3
123392	2	404291	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ongoing monitoring is essential for patients taking medicine for active tuberculosis .
	manualset3
123393	3	404291	13	NULL	NULL	0	NULL	medicine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Ongoing monitoring is essential for patients taking medicine for active tuberculosis .
	manualset3
123394	4	404291	13	NULL	NULL	0	NULL	tuberculosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Ongoing monitoring is essential for patients taking medicine for active tuberculosis .
	manualset3
123395	1	404292	13	NULL	NULL	0	NULL	14 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Only 14 patients required terminal care , three of whom received this entirely in hospital .
	manualset3
123396	2	404292	13	NULL	NULL	0	NULL	terminal care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Only 14 patients required terminal care , three of whom received this entirely in hospital .
	manualset3
123397	3	404292	13	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Only 14 patients required terminal care , three of whom received this entirely in hospital .
	manualset3
123398	4	404292	13	NULL	NULL	0	NULL	hospital	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Only 14 patients required terminal care , three of whom received this entirely in hospital .
	manualset3
123399	1	404293	13	NULL	NULL	0	NULL	concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Only a high concentration ( 10 ( -5 ) M ) of idazoxan was able to markedly antagonise the three contractile stimuli .
	manualset3
123400	2	404293	13	NULL	NULL	0	NULL	( 10 ( -5 ) M ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Only a high concentration ( 10 ( -5 ) M ) of idazoxan was able to markedly antagonise the three contractile stimuli .
	manualset3
123401	3	404293	13	NULL	NULL	0	NULL	idazoxan	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Only a high concentration ( 10 ( -5 ) M ) of idazoxan was able to markedly antagonise the three contractile stimuli .
	manualset3
123402	4	404293	13	NULL	NULL	0	NULL	three contractile stimuli	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Only a high concentration ( 10 ( -5 ) M ) of idazoxan was able to markedly antagonise the three contractile stimuli .
	manualset3
123437	1	404294	13	NULL	NULL	0	NULL	N-terminal peptide with 19 amino acid residues ( MAK19 ) 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Only an N-terminal peptide with 19 amino acid residues ( MAK19 ) showed cytotoxicity to the cell lines in dose - and time-dependent manners when introduced into cells by flanking the HIV-TAT protein transduction domain ( TAT-MAK19 ) .
	manualset3
123438	2	404294	13	NULL	NULL	0	NULL	cytotoxicity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Only an N-terminal peptide with 19 amino acid residues ( MAK19 ) showed cytotoxicity to the cell lines in dose - and time-dependent manners when introduced into cells by flanking the HIV-TAT protein transduction domain ( TAT-MAK19 ) .
	manualset3
123439	3	404294	13	NULL	NULL	0	NULL	cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Only an N-terminal peptide with 19 amino acid residues ( MAK19 ) showed cytotoxicity to the cell lines in dose - and time-dependent manners when introduced into cells by flanking the HIV-TAT protein transduction domain ( TAT-MAK19 ) .
	manualset3
123440	4	404294	13	NULL	NULL	0	NULL	dose-dependent manners	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Only an N-terminal peptide with 19 amino acid residues ( MAK19 ) showed cytotoxicity to the cell lines in dose - and time-dependent manners when introduced into cells by flanking the HIV-TAT protein transduction domain ( TAT-MAK19 ) .
	manualset3
123441	5	404294	13	NULL	NULL	0	NULL	time-dependent manners	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Only an N-terminal peptide with 19 amino acid residues ( MAK19 ) showed cytotoxicity to the cell lines in dose - and time-dependent manners when introduced into cells by flanking the HIV-TAT protein transduction domain ( TAT-MAK19 ) .
	manualset3
123442	6	404294	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Only an N-terminal peptide with 19 amino acid residues ( MAK19 ) showed cytotoxicity to the cell lines in dose - and time-dependent manners when introduced into cells by flanking the HIV-TAT protein transduction domain ( TAT-MAK19 ) .
	manualset3
123443	7	404294	13	NULL	NULL	0	NULL	HIV-TAT protein transduction domain ( TAT-MAK19 ) 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Only an N-terminal peptide with 19 amino acid residues ( MAK19 ) showed cytotoxicity to the cell lines in dose - and time-dependent manners when introduced into cells by flanking the HIV-TAT protein transduction domain ( TAT-MAK19 ) .
	manualset3
123444	1	404295	13	NULL	NULL	0	NULL	fractures 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Only fractures with total dislocation of the condyle out of the articulate fossa were surgically treated .
	manualset3
123445	2	404295	13	NULL	NULL	0	NULL	total dislocation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Only fractures with total dislocation of the condyle out of the articulate fossa were surgically treated .
	manualset3
123446	3	404295	13	NULL	NULL	0	NULL	condyle 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Only fractures with total dislocation of the condyle out of the articulate fossa were surgically treated .
	manualset3
123447	4	404295	13	NULL	NULL	0	NULL	articulate fossa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Only fractures with total dislocation of the condyle out of the articulate fossa were surgically treated .
	manualset3
123448	1	404296	13	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Only one child died during NR phase .
	manualset3
123449	2	404296	13	NULL	NULL	0	NULL	child	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Only one child died during NR phase .
	manualset3
123450	3	404296	13	NULL	NULL	0	NULL	NR phase	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Only one child died during NR phase .
	manualset3
123452	1	404297	13	NULL	NULL	0	NULL	one 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Only one individual whose dystonia developed in the setting of a measles infection carried the associated haplotype .
	manualset3
123453	2	404297	13	NULL	NULL	0	NULL	individual	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Only one individual whose dystonia developed in the setting of a measles infection carried the associated haplotype .
	manualset3
123454	3	404297	13	NULL	NULL	0	NULL	dystonia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Only one individual whose dystonia developed in the setting of a measles infection carried the associated haplotype .
	manualset3
123455	4	404297	13	NULL	NULL	0	NULL	setting	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Only one individual whose dystonia developed in the setting of a measles infection carried the associated haplotype .
	manualset3
123457	5	404297	13	NULL	NULL	0	NULL	measles infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Only one individual whose dystonia developed in the setting of a measles infection carried the associated haplotype .
	manualset3
123458	6	404297	13	NULL	NULL	0	NULL	haplotype 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Only one individual whose dystonia developed in the setting of a measles infection carried the associated haplotype .
	manualset3
123459	1	404298	13	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A direct relationship between renal arterial pressure ( RAP ) and cortical tissue nitric oxide ( NO ) activity in the canine kidney was reported earlier .
	manualset3
123460	2	404298	13	NULL	NULL	0	NULL	renal arterial pressure ( RAP ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A direct relationship between renal arterial pressure ( RAP ) and cortical tissue nitric oxide ( NO ) activity in the canine kidney was reported earlier .
	manualset3
123461	3	404298	13	NULL	NULL	0	NULL	cortical tissue nitric oxide ( NO ) activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A direct relationship between renal arterial pressure ( RAP ) and cortical tissue nitric oxide ( NO ) activity in the canine kidney was reported earlier .
	manualset3
123462	4	404298	13	NULL	NULL	0	NULL	canine kidney	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A direct relationship between renal arterial pressure ( RAP ) and cortical tissue nitric oxide ( NO ) activity in the canine kidney was reported earlier .
	manualset3
123464	1	404299	13	NULL	NULL	0	NULL	one 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Only one operation was unsuccessful and required conversion to conventional open laparotomy .
	manualset3
123465	2	404299	13	NULL	NULL	0	NULL	operation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Only one operation was unsuccessful and required conversion to conventional open laparotomy .
	manualset3
123466	3	404299	13	NULL	NULL	0	NULL	conversion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Only one operation was unsuccessful and required conversion to conventional open laparotomy .
	manualset3
123467	4	404299	13	NULL	NULL	0	NULL	open laparotomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Only one operation was unsuccessful and required conversion to conventional open laparotomy .
	manualset3
123470	1	404300	13	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Only one patient among recurrent aborters ( group one ) tested positive for abeta ( 2 ) GP-I .
	manualset3
123471	2	404300	13	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Only one patient among recurrent aborters ( group one ) tested positive for abeta ( 2 ) GP-I .
	manualset3
123472	3	404300	13	NULL	NULL	0	NULL	recurrent aborters ( group one )	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Only one patient among recurrent aborters ( group one ) tested positive for abeta ( 2 ) GP-I .
	manualset3
123473	4	404300	13	NULL	NULL	0	NULL	abeta ( 2 ) GP-I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Only one patient among recurrent aborters ( group one ) tested positive for abeta ( 2 ) GP-I .
	manualset3
123474	1	404301	13	NULL	NULL	0	NULL	protons	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Only protons ( primary and secondary ) were considered in the scoring of stopping-power .
	manualset3
123475	2	404301	13	NULL	NULL	0	NULL	scoring	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Only protons ( primary and secondary ) were considered in the scoring of stopping-power .
	manualset3
123476	3	404301	13	NULL	NULL	0	NULL	stopping-power	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Only protons ( primary and secondary ) were considered in the scoring of stopping-power .
	manualset3
123478	1	404302	13	NULL	NULL	0	NULL	DNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Only the DNA of the strains isolated from soil in Scotland and the United States and that of five of the New Caledonian strains did not show any detectable homologies to any of our probes .
	manualset3
123480	2	404302	13	NULL	NULL	0	NULL	strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Only the DNA of the strains isolated from soil in Scotland and the United States and that of five of the New Caledonian strains did not show any detectable homologies to any of our probes .
	manualset3
123482	3	404302	13	NULL	NULL	0	NULL	soil	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Only the DNA of the strains isolated from soil in Scotland and the United States and that of five of the New Caledonian strains did not show any detectable homologies to any of our probes .
	manualset3
123484	4	404302	13	NULL	NULL	0	NULL	Scotland	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Only the DNA of the strains isolated from soil in Scotland and the United States and that of five of the New Caledonian strains did not show any detectable homologies to any of our probes .
	manualset3
123485	5	404302	13	NULL	NULL	0	NULL	United States	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Only the DNA of the strains isolated from soil in Scotland and the United States and that of five of the New Caledonian strains did not show any detectable homologies to any of our probes .
	manualset3
123486	6	404302	13	NULL	NULL	0	NULL	five 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Only the DNA of the strains isolated from soil in Scotland and the United States and that of five of the New Caledonian strains did not show any detectable homologies to any of our probes .
	manualset3
123487	7	404302	13	NULL	NULL	0	NULL	New Caledonian strains 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Only the DNA of the strains isolated from soil in Scotland and the United States and that of five of the New Caledonian strains did not show any detectable homologies to any of our probes .
	manualset3
123488	8	404302	13	NULL	NULL	0	NULL	detectable homologies	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Only the DNA of the strains isolated from soil in Scotland and the United States and that of five of the New Caledonian strains did not show any detectable homologies to any of our probes .
	manualset3
123489	9	404302	13	NULL	NULL	0	NULL	probes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Only the DNA of the strains isolated from soil in Scotland and the United States and that of five of the New Caledonian strains did not show any detectable homologies to any of our probes .
	manualset3
123490	1	404303	13	NULL	NULL	0	NULL	radiation dose 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Only the highest radiation dose given , 375 rad per day to a total of 11 , 250 rad , resulted in a complete response rate and tumor cure rate of 50 % when CP was added .
	manualset3
123491	2	404303	13	NULL	NULL	0	NULL	375 rad per day	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Only the highest radiation dose given , 375 rad per day to a total of 11 , 250 rad , resulted in a complete response rate and tumor cure rate of 50 % when CP was added .
	manualset3
123492	3	404303	13	NULL	NULL	0	NULL	total of 11 , 250 rad	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Only the highest radiation dose given , 375 rad per day to a total of 11 , 250 rad , resulted in a complete response rate and tumor cure rate of 50 % when CP was added .
	manualset3
123493	4	404303	13	NULL	NULL	0	NULL	complete response rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Only the highest radiation dose given , 375 rad per day to a total of 11 , 250 rad , resulted in a complete response rate and tumor cure rate of 50 % when CP was added .
	manualset3
123494	5	404303	13	NULL	NULL	0	NULL	tumor cure rate 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Only the highest radiation dose given , 375 rad per day to a total of 11 , 250 rad , resulted in a complete response rate and tumor cure rate of 50 % when CP was added .
	manualset3
123495	6	404303	13	NULL	NULL	0	NULL	50 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Only the highest radiation dose given , 375 rad per day to a total of 11 , 250 rad , resulted in a complete response rate and tumor cure rate of 50 % when CP was added .
	manualset3
123496	7	404303	13	NULL	NULL	0	NULL	CP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Only the highest radiation dose given , 375 rad per day to a total of 11 , 250 rad , resulted in a complete response rate and tumor cure rate of 50 % when CP was added .
	manualset3
123497	1	404304	13	NULL	NULL	0	NULL	proximal GnRH1-responsive region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Only the proximal GnRH1-responsive region of the promoter was required for cAMP stimulation , and mutation of the 3 ' NR5A1 site diminished the response .
	manualset3
123498	2	404304	13	NULL	NULL	0	NULL	promoter 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Only the proximal GnRH1-responsive region of the promoter was required for cAMP stimulation , and mutation of the 3 ' NR5A1 site diminished the response .
	manualset3
123501	3	404304	13	NULL	NULL	NULL	NULL	cAMP stimulation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Only the proximal GnRH1-responsive region of the promoter was required for cAMP stimulation , and mutation of the 3 ' NR5A1 site diminished the response .
	manualset3
123503	4	404304	13	NULL	NULL	0	NULL	mutation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Only the proximal GnRH1-responsive region of the promoter was required for cAMP stimulation , and mutation of the 3 ' NR5A1 site diminished the response .
	manualset3
123505	5	404304	13	NULL	NULL	0	NULL	3 ' NR5A1 site	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Only the proximal GnRH1-responsive region of the promoter was required for cAMP stimulation , and mutation of the 3 ' NR5A1 site diminished the response .
	manualset3
123507	6	404304	13	NULL	NULL	NULL	NULL	response	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Only the proximal GnRH1-responsive region of the promoter was required for cAMP stimulation , and mutation of the 3 ' NR5A1 site diminished the response .
	manualset3
123508	1	404305	13	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A direct relationship was observed between the change in chemical shift ( ( delta delta ) of the 2-P and 3-P of diphosphoglycerate and the percent diphosphoglycerate bound , when the latter was varied by altering pH , oxygenation state , or total diphosphoglycerate concentration .
	manualset3
123509	2	404305	13	NULL	NULL	0	NULL	change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A direct relationship was observed between the change in chemical shift ( ( delta delta ) of the 2-P and 3-P of diphosphoglycerate and the percent diphosphoglycerate bound , when the latter was varied by altering pH , oxygenation state , or total diphosphoglycerate concentration .
	manualset3
123512	3	404305	13	NULL	NULL	0	NULL	chemical shift	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A direct relationship was observed between the change in chemical shift ( ( delta delta ) of the 2-P and 3-P of diphosphoglycerate and the percent diphosphoglycerate bound , when the latter was varied by altering pH , oxygenation state , or total diphosphoglycerate concentration .
	manualset3
123513	4	404305	13	NULL	NULL	0	NULL	( ( delta delta ) of the 2-P and 3-P of diphosphoglycerate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A direct relationship was observed between the change in chemical shift ( ( delta delta ) of the 2-P and 3-P of diphosphoglycerate and the percent diphosphoglycerate bound , when the latter was varied by altering pH , oxygenation state , or total diphosphoglycerate concentration .
	manualset3
123514	5	404305	13	NULL	NULL	0	NULL	percent 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A direct relationship was observed between the change in chemical shift ( ( delta delta ) of the 2-P and 3-P of diphosphoglycerate and the percent diphosphoglycerate bound , when the latter was varied by altering pH , oxygenation state , or total diphosphoglycerate concentration .
	manualset3
123515	6	404305	13	NULL	NULL	0	NULL	diphosphoglycerate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A direct relationship was observed between the change in chemical shift ( ( delta delta ) of the 2-P and 3-P of diphosphoglycerate and the percent diphosphoglycerate bound , when the latter was varied by altering pH , oxygenation state , or total diphosphoglycerate concentration .
	manualset3
123516	7	404305	13	NULL	NULL	NULL	NULL	pH	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A direct relationship was observed between the change in chemical shift ( ( delta delta ) of the 2-P and 3-P of diphosphoglycerate and the percent diphosphoglycerate bound , when the latter was varied by altering pH , oxygenation state , or total diphosphoglycerate concentration .
	manualset3
123518	8	404305	13	NULL	NULL	0	NULL	oxygenation state	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A direct relationship was observed between the change in chemical shift ( ( delta delta ) of the 2-P and 3-P of diphosphoglycerate and the percent diphosphoglycerate bound , when the latter was varied by altering pH , oxygenation state , or total diphosphoglycerate concentration .
	manualset3
123519	9	404305	13	NULL	NULL	0	NULL	total diphosphoglycerate concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A direct relationship was observed between the change in chemical shift ( ( delta delta ) of the 2-P and 3-P of diphosphoglycerate and the percent diphosphoglycerate bound , when the latter was varied by altering pH , oxygenation state , or total diphosphoglycerate concentration .
	manualset3
123528	1	404306	13	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Only two isolates E-45 and E-65 significantly inhibited the in vitro growth of Ecc P-138 .
	manualset3
123530	2	404306	13	NULL	NULL	0	NULL	E-45	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Only two isolates E-45 and E-65 significantly inhibited the in vitro growth of Ecc P-138 .
	manualset3
123531	3	404306	13	NULL	NULL	0	NULL	E-65	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Only two isolates E-45 and E-65 significantly inhibited the in vitro growth of Ecc P-138 .
	manualset3
123534	4	404306	13	NULL	NULL	0	NULL	growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Only two isolates E-45 and E-65 significantly inhibited the in vitro growth of Ecc P-138 .
	manualset3
123535	5	404306	13	NULL	NULL	0	NULL	Ecc P-138	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Only two isolates E-45 and E-65 significantly inhibited the in vitro growth of Ecc P-138 .
	manualset3
123537	1	404307	13	NULL	NULL	0	NULL	conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Only under conditions where the inner membrane was accessible to the probe , Gut2p was labeled by ( 125I ) TID-PC , in parallel with increased labeling of the phosphate carrier ( P ( i ) C ) in the inner membrane .
	manualset3
123538	2	404307	13	NULL	NULL	0	NULL	inner membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Only under conditions where the inner membrane was accessible to the probe , Gut2p was labeled by ( 125I ) TID-PC , in parallel with increased labeling of the phosphate carrier ( P ( i ) C ) in the inner membrane .
	manualset3
123539	3	404307	13	NULL	NULL	0	NULL	probe	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Only under conditions where the inner membrane was accessible to the probe , Gut2p was labeled by ( 125I ) TID-PC , in parallel with increased labeling of the phosphate carrier ( P ( i ) C ) in the inner membrane .
	manualset3
123540	4	404307	13	NULL	NULL	0	NULL	Gut2p	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Only under conditions where the inner membrane was accessible to the probe , Gut2p was labeled by ( 125I ) TID-PC , in parallel with increased labeling of the phosphate carrier ( P ( i ) C ) in the inner membrane .
	manualset3
123541	5	404307	13	NULL	NULL	0	NULL	( 125I ) TID-PC	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Only under conditions where the inner membrane was accessible to the probe , Gut2p was labeled by ( 125I ) TID-PC , in parallel with increased labeling of the phosphate carrier ( P ( i ) C ) in the inner membrane .
	manualset3
123543	6	404307	13	NULL	NULL	0	NULL	 phosphate carrier ( P ( i ) C )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Only under conditions where the inner membrane was accessible to the probe , Gut2p was labeled by ( 125I ) TID-PC , in parallel with increased labeling of the phosphate carrier ( P ( i ) C ) in the inner membrane .
	manualset3
123545	7	404307	13	NULL	NULL	0	NULL	inner membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Only under conditions where the inner membrane was accessible to the probe , Gut2p was labeled by ( 125I ) TID-PC , in parallel with increased labeling of the phosphate carrier ( P ( i ) C ) in the inner membrane .
	manualset3
123548	1	404308	13	NULL	NULL	0	NULL	Onset of scoliosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Onset of scoliosis averaged 8.8 years .
	manualset3
123549	2	404308	13	NULL	NULL	0	NULL	8.8 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Onset of scoliosis averaged 8.8 years .
	manualset3
123550	1	404309	13	NULL	NULL	NULL	NULL	Ontogenetic development 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ontogenetic development of synovial A cells in fetal and neonatal rat knee joints .
	manualset3
123551	2	404309	13	NULL	NULL	0	NULL	synovial A cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Ontogenetic development of synovial A cells in fetal and neonatal rat knee joints .
	manualset3
123552	3	404309	13	NULL	NULL	0	NULL	fetal rat knee joints	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ontogenetic development of synovial A cells in fetal and neonatal rat knee joints .
	manualset3
123553	4	404309	13	NULL	NULL	0	NULL	neonatal rat knee joints 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ontogenetic development of synovial A cells in fetal and neonatal rat knee joints .
	manualset3
123554	1	404310	13	NULL	NULL	0	NULL	Ontogenic origin	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ontogenic origin of salmon GnRH neurons in the ventral telencephalon and the preoptic area in masu salmon .
	manualset3
123555	2	404310	13	NULL	NULL	0	NULL	salmon GnRH neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Ontogenic origin of salmon GnRH neurons in the ventral telencephalon and the preoptic area in masu salmon .
	manualset3
123556	3	404310	13	NULL	NULL	0	NULL	ventral telencephalon	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ontogenic origin of salmon GnRH neurons in the ventral telencephalon and the preoptic area in masu salmon .
	manualset3
123557	4	404310	13	NULL	NULL	0	NULL	preoptic area	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ontogenic origin of salmon GnRH neurons in the ventral telencephalon and the preoptic area in masu salmon .
	manualset3
123558	5	404310	13	NULL	NULL	0	NULL	masu salmon	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ontogenic origin of salmon GnRH neurons in the ventral telencephalon and the preoptic area in masu salmon .
	manualset3
123559	1	404311	13	NULL	NULL	0	NULL	Open heart operation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Open heart operation in a patient with hereditary spherocytosis : a case report .
	manualset3
123560	2	404311	13	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Open heart operation in a patient with hereditary spherocytosis : a case report .
	manualset3
123561	3	404311	13	NULL	NULL	0	NULL	 hereditary spherocytosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Open heart operation in a patient with hereditary spherocytosis : a case report .
	manualset3
123562	4	404311	13	NULL	NULL	0	NULL	case report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Open heart operation in a patient with hereditary spherocytosis : a case report .
	manualset3
123563	1	404312	13	NULL	NULL	0	NULL	Openings 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Openings between these cells contribute to tumor vessel leakiness and may permit access of macromolecular therapeutic agents to tumor cells .
	manualset3
123564	2	404312	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Openings between these cells contribute to tumor vessel leakiness and may permit access of macromolecular therapeutic agents to tumor cells .
	manualset3
123565	3	404312	13	NULL	NULL	0	NULL	tumor vessel leakiness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Openings between these cells contribute to tumor vessel leakiness and may permit access of macromolecular therapeutic agents to tumor cells .
	manualset3
123566	4	404312	13	NULL	NULL	0	NULL	access	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Openings between these cells contribute to tumor vessel leakiness and may permit access of macromolecular therapeutic agents to tumor cells .
	manualset3
123567	5	404312	13	NULL	NULL	NULL	NULL	macromolecular therapeutic agents 	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Openings between these cells contribute to tumor vessel leakiness and may permit access of macromolecular therapeutic agents to tumor cells .
	manualset3
123568	6	404312	13	NULL	NULL	0	NULL	tumor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Openings between these cells contribute to tumor vessel leakiness and may permit access of macromolecular therapeutic agents to tumor cells .
	manualset3
123569	1	404313	13	NULL	NULL	0	NULL	discontinuity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A discontinuity in the activation barrier for the chemical reaction is not expected in the transition temperature range .
	manualset3
123570	2	404313	13	NULL	NULL	0	NULL	activation barrier	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A discontinuity in the activation barrier for the chemical reaction is not expected in the transition temperature range .
	manualset3
123571	3	404313	13	NULL	NULL	0	NULL	chemical reaction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A discontinuity in the activation barrier for the chemical reaction is not expected in the transition temperature range .
	manualset3
123572	4	404313	13	NULL	NULL	0	NULL	transition temperature range	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A discontinuity in the activation barrier for the chemical reaction is not expected in the transition temperature range .
	manualset3
123573	1	404314	13	NULL	NULL	0	NULL	Operation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Operation confirmed the angiographic findings , particularly the independent nature of the mass i relation to the kidney and the excretory pathways .
	manualset3
123574	2	404314	13	NULL	NULL	0	NULL	angiographic findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Operation confirmed the angiographic findings , particularly the independent nature of the mass i relation to the kidney and the excretory pathways .
	manualset3
123575	3	404314	13	NULL	NULL	0	NULL	nature 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Operation confirmed the angiographic findings , particularly the independent nature of the mass i relation to the kidney and the excretory pathways .
	manualset3
123576	4	404314	13	NULL	NULL	0	NULL	mass i relation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Operation confirmed the angiographic findings , particularly the independent nature of the mass i relation to the kidney and the excretory pathways .
	manualset3
123577	5	404314	13	NULL	NULL	0	NULL	kidney pathways	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Operation confirmed the angiographic findings , particularly the independent nature of the mass i relation to the kidney and the excretory pathways .
	manualset3
123578	6	404314	13	NULL	NULL	0	NULL	excretory pathways	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Operation confirmed the angiographic findings , particularly the independent nature of the mass i relation to the kidney and the excretory pathways .
	manualset3
123579	1	404315	13	NULL	NULL	0	NULL	Operational use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Operational use of the United States Air Force partial pressure suit .
	manualset3
123580	2	404315	13	NULL	NULL	0	NULL	United States	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Operational use of the United States Air Force partial pressure suit .
	manualset3
123581	3	404315	13	NULL	NULL	0	NULL	Air Force partial pressure suit	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Operational use of the United States Air Force partial pressure suit .
	manualset3
123598	1	404316	13	NULL	NULL	0	NULL	Operations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Operations performed were ( 1 ) longitudinal arteriotomy through the stent with patch angioplasty , ( 2 ) common carotid to distal internal carotid artery ( ICA ) bypass with polytetrafluoroethylene ( PTFE ) , ( 3 ) subclavian to distal ICA bypass with PTFE , and ( 4 ) carotid endarterectomy with complete stent removal and patch angioplasty .
	manualset3
123599	2	404316	13	NULL	NULL	0	NULL	longitudinal arteriotomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Operations performed were ( 1 ) longitudinal arteriotomy through the stent with patch angioplasty , ( 2 ) common carotid to distal internal carotid artery ( ICA ) bypass with polytetrafluoroethylene ( PTFE ) , ( 3 ) subclavian to distal ICA bypass with PTFE , and ( 4 ) carotid endarterectomy with complete stent removal and patch angioplasty .
	manualset3
123600	3	404316	13	NULL	NULL	0	NULL	stent	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Operations performed were ( 1 ) longitudinal arteriotomy through the stent with patch angioplasty , ( 2 ) common carotid to distal internal carotid artery ( ICA ) bypass with polytetrafluoroethylene ( PTFE ) , ( 3 ) subclavian to distal ICA bypass with PTFE , and ( 4 ) carotid endarterectomy with complete stent removal and patch angioplasty .
	manualset3
123601	4	404316	13	NULL	NULL	0	NULL	patch angioplasty	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Operations performed were ( 1 ) longitudinal arteriotomy through the stent with patch angioplasty , ( 2 ) common carotid to distal internal carotid artery ( ICA ) bypass with polytetrafluoroethylene ( PTFE ) , ( 3 ) subclavian to distal ICA bypass with PTFE , and ( 4 ) carotid endarterectomy with complete stent removal and patch angioplasty .
	manualset3
123602	5	404316	13	NULL	NULL	0	NULL	common carotid to distal internal carotid artery ( ICA ) bypass	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Operations performed were ( 1 ) longitudinal arteriotomy through the stent with patch angioplasty , ( 2 ) common carotid to distal internal carotid artery ( ICA ) bypass with polytetrafluoroethylene ( PTFE ) , ( 3 ) subclavian to distal ICA bypass with PTFE , and ( 4 ) carotid endarterectomy with complete stent removal and patch angioplasty .
	manualset3
123603	6	404316	13	NULL	NULL	0	NULL	polytetrafluoroethylene ( PTFE ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Operations performed were ( 1 ) longitudinal arteriotomy through the stent with patch angioplasty , ( 2 ) common carotid to distal internal carotid artery ( ICA ) bypass with polytetrafluoroethylene ( PTFE ) , ( 3 ) subclavian to distal ICA bypass with PTFE , and ( 4 ) carotid endarterectomy with complete stent removal and patch angioplasty .
	manualset3
123604	7	404316	13	NULL	NULL	0	NULL	subclavian to distal ICA bypass	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Operations performed were ( 1 ) longitudinal arteriotomy through the stent with patch angioplasty , ( 2 ) common carotid to distal internal carotid artery ( ICA ) bypass with polytetrafluoroethylene ( PTFE ) , ( 3 ) subclavian to distal ICA bypass with PTFE , and ( 4 ) carotid endarterectomy with complete stent removal and patch angioplasty .
	manualset3
123605	8	404316	13	NULL	NULL	0	NULL	PTFE	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Operations performed were ( 1 ) longitudinal arteriotomy through the stent with patch angioplasty , ( 2 ) common carotid to distal internal carotid artery ( ICA ) bypass with polytetrafluoroethylene ( PTFE ) , ( 3 ) subclavian to distal ICA bypass with PTFE , and ( 4 ) carotid endarterectomy with complete stent removal and patch angioplasty .
	manualset3
123606	9	404316	13	NULL	NULL	0	NULL	 carotid endarterectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Operations performed were ( 1 ) longitudinal arteriotomy through the stent with patch angioplasty , ( 2 ) common carotid to distal internal carotid artery ( ICA ) bypass with polytetrafluoroethylene ( PTFE ) , ( 3 ) subclavian to distal ICA bypass with PTFE , and ( 4 ) carotid endarterectomy with complete stent removal and patch angioplasty .
	manualset3
123607	10	404316	13	NULL	NULL	0	NULL	stent 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Operations performed were ( 1 ) longitudinal arteriotomy through the stent with patch angioplasty , ( 2 ) common carotid to distal internal carotid artery ( ICA ) bypass with polytetrafluoroethylene ( PTFE ) , ( 3 ) subclavian to distal ICA bypass with PTFE , and ( 4 ) carotid endarterectomy with complete stent removal and patch angioplasty .
	manualset3
123608	11	404316	13	NULL	NULL	0	NULL	patch angioplasty	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Operations performed were ( 1 ) longitudinal arteriotomy through the stent with patch angioplasty , ( 2 ) common carotid to distal internal carotid artery ( ICA ) bypass with polytetrafluoroethylene ( PTFE ) , ( 3 ) subclavian to distal ICA bypass with PTFE , and ( 4 ) carotid endarterectomy with complete stent removal and patch angioplasty .
	manualset3
123596	1	404317	13	NULL	NULL	0	NULL	Operative note dictation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Operative note dictation : should it be taught routinely in residency programs ?
	manualset3
123597	2	404317	13	NULL	NULL	0	NULL	residency programs	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Operative note dictation : should it be taught routinely in residency programs ?
	manualset3
123591	1	404318	13	NULL	NULL	0	NULL	Opinions 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Opinions were generally favorable ; most users felt that CP makes their work more accurate , reduces errors , is easy to learn and to use , and provides important and useful information .
	manualset3
123592	2	404318	13	NULL	NULL	0	NULL	users 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Opinions were generally favorable ; most users felt that CP makes their work more accurate , reduces errors , is easy to learn and to use , and provides important and useful information .
	manualset3
123593	3	404318	13	NULL	NULL	0	NULL	CP	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Opinions were generally favorable ; most users felt that CP makes their work more accurate , reduces errors , is easy to learn and to use , and provides important and useful information .
	manualset3
123594	4	404318	13	NULL	NULL	NULL	NULL	errors	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Opinions were generally favorable ; most users felt that CP makes their work more accurate , reduces errors , is easy to learn and to use , and provides important and useful information .
	manualset3
123595	5	404318	13	NULL	NULL	0	NULL	useful information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Opinions were generally favorable ; most users felt that CP makes their work more accurate , reduces errors , is easy to learn and to use , and provides important and useful information .
	manualset3
123588	1	404319	13	NULL	NULL	0	NULL	Opioid addiction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Opioid addiction and incarceration : an overview .
	manualset3
123589	2	404319	13	NULL	NULL	0	NULL	incarceration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Opioid addiction and incarceration : an overview .
	manualset3
123590	3	404319	13	NULL	NULL	0	NULL	overview	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Opioid addiction and incarceration : an overview .
	manualset3
123582	1	404320	13	NULL	NULL	0	NULL	Optic-morphological characteristics 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Optic-morphological characteristics and crystallization of mucus of land snails Achatina fulica ( Bowditch ) are compared with cervical secret and also with the human bile .
	manualset3
123583	2	404320	13	NULL	NULL	0	NULL	crystallization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Optic-morphological characteristics and crystallization of mucus of land snails Achatina fulica ( Bowditch ) are compared with cervical secret and also with the human bile .
	manualset3
123584	3	404320	13	NULL	NULL	0	NULL	mucus 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Optic-morphological characteristics and crystallization of mucus of land snails Achatina fulica ( Bowditch ) are compared with cervical secret and also with the human bile .
	manualset3
123585	4	404320	13	NULL	NULL	0	NULL	land snails Achatina fulica ( Bowditch ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Optic-morphological characteristics and crystallization of mucus of land snails Achatina fulica ( Bowditch ) are compared with cervical secret and also with the human bile .
	manualset3
123586	5	404320	13	NULL	NULL	0	NULL	cervical secret	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Optic-morphological characteristics and crystallization of mucus of land snails Achatina fulica ( Bowditch ) are compared with cervical secret and also with the human bile .
	manualset3
123587	6	404320	13	NULL	NULL	0	NULL	human bile	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Optic-morphological characteristics and crystallization of mucus of land snails Achatina fulica ( Bowditch ) are compared with cervical secret and also with the human bile .
	manualset3
123828	1	404321	13	NULL	NULL	0	NULL	Optical designs 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Optical designs of aspheric internally reflective concentrators of divergent light emitted within a spatial angle of 2n sr are proposed and discussed .
	manualset3
123829	2	404321	13	NULL	NULL	0	NULL	concentrators	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Optical designs of aspheric internally reflective concentrators of divergent light emitted within a spatial angle of 2n sr are proposed and discussed .
	manualset3
123830	3	404321	13	NULL	NULL	0	NULL	light	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Optical designs of aspheric internally reflective concentrators of divergent light emitted within a spatial angle of 2n sr are proposed and discussed .
	manualset3
123831	4	404321	13	NULL	NULL	0	NULL	spatial angle	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Optical designs of aspheric internally reflective concentrators of divergent light emitted within a spatial angle of 2n sr are proposed and discussed .
	manualset3
123832	5	404321	13	NULL	NULL	0	NULL	 2n sr	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Optical designs of aspheric internally reflective concentrators of divergent light emitted within a spatial angle of 2n sr are proposed and discussed .
	manualset3
123833	1	404322	13	NULL	NULL	0	NULL	discussion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A discussion and recommendations on chemical analyses of rosin components follow .
	manualset3
123834	2	404322	13	NULL	NULL	0	NULL	recommendations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A discussion and recommendations on chemical analyses of rosin components follow .
	manualset3
123835	3	404322	13	NULL	NULL	0	NULL	chemical analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A discussion and recommendations on chemical analyses of rosin components follow .
	manualset3
123836	4	404322	13	NULL	NULL	0	NULL	rosin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A discussion and recommendations on chemical analyses of rosin components follow .
	manualset3
123837	1	404323	13	NULL	NULL	0	NULL	Optical distortion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Optical distortion due to pulses having durations on the order of the acoustic wave propagation time through the thickness of the window is a result of heating by the absorbed laser energy and thermally induced plane-strain stress waves .
	manualset3
123838	2	404323	13	NULL	NULL	0	NULL	pulses	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Optical distortion due to pulses having durations on the order of the acoustic wave propagation time through the thickness of the window is a result of heating by the absorbed laser energy and thermally induced plane-strain stress waves .
	manualset3
123839	3	404323	13	NULL	NULL	0	NULL	durations	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Optical distortion due to pulses having durations on the order of the acoustic wave propagation time through the thickness of the window is a result of heating by the absorbed laser energy and thermally induced plane-strain stress waves .
	manualset3
123840	4	404323	13	NULL	NULL	0	NULL	order	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Optical distortion due to pulses having durations on the order of the acoustic wave propagation time through the thickness of the window is a result of heating by the absorbed laser energy and thermally induced plane-strain stress waves .
	manualset3
123841	5	404323	13	NULL	NULL	0	NULL	acoustic wave propagation time 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Optical distortion due to pulses having durations on the order of the acoustic wave propagation time through the thickness of the window is a result of heating by the absorbed laser energy and thermally induced plane-strain stress waves .
	manualset3
123842	6	404323	13	NULL	NULL	0	NULL	thickness	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Optical distortion due to pulses having durations on the order of the acoustic wave propagation time through the thickness of the window is a result of heating by the absorbed laser energy and thermally induced plane-strain stress waves .
	manualset3
123843	7	404323	13	NULL	NULL	0	NULL	window	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Optical distortion due to pulses having durations on the order of the acoustic wave propagation time through the thickness of the window is a result of heating by the absorbed laser energy and thermally induced plane-strain stress waves .
	manualset3
123844	8	404323	13	NULL	NULL	0	NULL	result	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Optical distortion due to pulses having durations on the order of the acoustic wave propagation time through the thickness of the window is a result of heating by the absorbed laser energy and thermally induced plane-strain stress waves .
	manualset3
123845	9	404323	13	NULL	NULL	0	NULL	heating 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Optical distortion due to pulses having durations on the order of the acoustic wave propagation time through the thickness of the window is a result of heating by the absorbed laser energy and thermally induced plane-strain stress waves .
	manualset3
123846	10	404323	13	NULL	NULL	0	NULL	laser energy	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Optical distortion due to pulses having durations on the order of the acoustic wave propagation time through the thickness of the window is a result of heating by the absorbed laser energy and thermally induced plane-strain stress waves .
	manualset3
123847	11	404323	13	NULL	NULL	0	NULL	plane-strain stress waves	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Optical distortion due to pulses having durations on the order of the acoustic wave propagation time through the thickness of the window is a result of heating by the absorbed laser energy and thermally induced plane-strain stress waves .
	manualset3
123848	1	404324	13	NULL	NULL	0	NULL	Optimal binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal binding of hirudin to thrombin occurred when the groups with pKa values of 8.4 and 9.0 were protonated and the other group with a pKa of 7.1 was deprotonated .
	manualset3
123849	2	404324	13	NULL	NULL	0	NULL	hirudin	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal binding of hirudin to thrombin occurred when the groups with pKa values of 8.4 and 9.0 were protonated and the other group with a pKa of 7.1 was deprotonated .
	manualset3
123858	3	404324	13	NULL	NULL	0	NULL	thrombin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal binding of hirudin to thrombin occurred when the groups with pKa values of 8.4 and 9.0 were protonated and the other group with a pKa of 7.1 was deprotonated .
	manualset3
123864	4	404324	13	NULL	NULL	0	NULL	groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal binding of hirudin to thrombin occurred when the groups with pKa values of 8.4 and 9.0 were protonated and the other group with a pKa of 7.1 was deprotonated .
	manualset3
123866	5	404324	13	NULL	NULL	0	NULL	pKa values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal binding of hirudin to thrombin occurred when the groups with pKa values of 8.4 and 9.0 were protonated and the other group with a pKa of 7.1 was deprotonated .
	manualset3
123867	6	404324	13	NULL	NULL	0	NULL	8.4	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal binding of hirudin to thrombin occurred when the groups with pKa values of 8.4 and 9.0 were protonated and the other group with a pKa of 7.1 was deprotonated .
	manualset3
123868	7	404324	13	NULL	NULL	0	NULL	9.0	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal binding of hirudin to thrombin occurred when the groups with pKa values of 8.4 and 9.0 were protonated and the other group with a pKa of 7.1 was deprotonated .
	manualset3
123869	8	404324	13	NULL	NULL	0	NULL	group	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal binding of hirudin to thrombin occurred when the groups with pKa values of 8.4 and 9.0 were protonated and the other group with a pKa of 7.1 was deprotonated .
	manualset3
123870	9	404324	13	NULL	NULL	0	NULL	pKa	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal binding of hirudin to thrombin occurred when the groups with pKa values of 8.4 and 9.0 were protonated and the other group with a pKa of 7.1 was deprotonated .
	manualset3
123871	10	404324	13	NULL	NULL	0	NULL	7.1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal binding of hirudin to thrombin occurred when the groups with pKa values of 8.4 and 9.0 were protonated and the other group with a pKa of 7.1 was deprotonated .
	manualset3
123876	1	404325	13	NULL	NULL	0	NULL	Optimal conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal conditions are achieved with end-to-end or side-to-side anastomoses of single organs ( for example between small bowel and small bowel or colon and colon ) .
	manualset3
123883	2	404325	13	NULL	NULL	0	NULL	end-to-end anastomoses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal conditions are achieved with end-to-end or side-to-side anastomoses of single organs ( for example between small bowel and small bowel or colon and colon ) .
	manualset3
123884	3	404325	13	NULL	NULL	NULL	NULL	side-to-side anastomoses	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Optimal conditions are achieved with end-to-end or side-to-side anastomoses of single organs ( for example between small bowel and small bowel or colon and colon ) .
	manualset3
123886	4	404325	13	NULL	NULL	0	NULL	single organs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal conditions are achieved with end-to-end or side-to-side anastomoses of single organs ( for example between small bowel and small bowel or colon and colon ) .
	manualset3
123888	5	404325	13	NULL	NULL	NULL	NULL	example	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Optimal conditions are achieved with end-to-end or side-to-side anastomoses of single organs ( for example between small bowel and small bowel or colon and colon ) .
	manualset3
123889	6	404325	13	NULL	NULL	0	NULL	small bowel 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal conditions are achieved with end-to-end or side-to-side anastomoses of single organs ( for example between small bowel and small bowel or colon and colon ) .
	manualset3
123897	7	404325	13	NULL	NULL	0	NULL	small bowel	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal conditions are achieved with end-to-end or side-to-side anastomoses of single organs ( for example between small bowel and small bowel or colon and colon ) .
	manualset3
123899	8	404325	13	NULL	NULL	0	NULL	colon	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal conditions are achieved with end-to-end or side-to-side anastomoses of single organs ( for example between small bowel and small bowel or colon and colon ) .
	manualset3
123901	9	404325	13	NULL	NULL	0	NULL	colon	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal conditions are achieved with end-to-end or side-to-side anastomoses of single organs ( for example between small bowel and small bowel or colon and colon ) .
	manualset3
123908	1	404326	13	NULL	NULL	0	NULL	Optimal correlations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal correlations were found between the probit transform of the drug-induced increased lifespan ( ILS ) and field and pi parameters .
	manualset3
123909	2	404326	13	NULL	NULL	0	NULL	probit	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal correlations were found between the probit transform of the drug-induced increased lifespan ( ILS ) and field and pi parameters .
	manualset3
123910	3	404326	13	NULL	NULL	0	NULL	lifespan ( ILS )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal correlations were found between the probit transform of the drug-induced increased lifespan ( ILS ) and field and pi parameters .
	manualset3
123911	4	404326	13	NULL	NULL	0	NULL	field parameters	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal correlations were found between the probit transform of the drug-induced increased lifespan ( ILS ) and field and pi parameters .
	manualset3
123912	5	404326	13	NULL	NULL	0	NULL	pi parameters	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal correlations were found between the probit transform of the drug-induced increased lifespan ( ILS ) and field and pi parameters .
	manualset3
123913	1	404327	13	NULL	NULL	0	NULL	Optimal outcomes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal outcomes for liver-dominant metastatic breast cancer with transarterial chemoembolization with drug-eluting beads loaded with doxorubicin .
	manualset3
123914	2	404327	13	NULL	NULL	0	NULL	liver-dominant metastatic breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal outcomes for liver-dominant metastatic breast cancer with transarterial chemoembolization with drug-eluting beads loaded with doxorubicin .
	manualset3
123915	3	404327	13	NULL	NULL	0	NULL	transarterial chemoembolization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal outcomes for liver-dominant metastatic breast cancer with transarterial chemoembolization with drug-eluting beads loaded with doxorubicin .
	manualset3
123916	4	404327	13	NULL	NULL	0	NULL	drug-eluting beads	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal outcomes for liver-dominant metastatic breast cancer with transarterial chemoembolization with drug-eluting beads loaded with doxorubicin .
	manualset3
123917	5	404327	13	NULL	NULL	0	NULL	doxorubicin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal outcomes for liver-dominant metastatic breast cancer with transarterial chemoembolization with drug-eluting beads loaded with doxorubicin .
	manualset3
123918	1	404328	13	NULL	NULL	0	NULL	Optimal risk factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal risk factors in the population : prognosis , prevalence , and secular trends ; data from Gteborg population studies .
	manualset3
123919	2	404328	13	NULL	NULL	0	NULL	population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal risk factors in the population : prognosis , prevalence , and secular trends ; data from Gteborg population studies .
	manualset3
123921	3	404328	13	NULL	NULL	0	NULL	prognosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal risk factors in the population : prognosis , prevalence , and secular trends ; data from Gteborg population studies .
	manualset3
123922	4	404328	13	NULL	NULL	0	NULL	prevalence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal risk factors in the population : prognosis , prevalence , and secular trends ; data from Gteborg population studies .
	manualset3
123923	5	404328	13	NULL	NULL	0	NULL	secular trends	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal risk factors in the population : prognosis , prevalence , and secular trends ; data from Gteborg population studies .
	manualset3
123924	6	404328	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal risk factors in the population : prognosis , prevalence , and secular trends ; data from Gteborg population studies .
	manualset3
123925	7	404328	13	NULL	NULL	0	NULL	Gteborg population studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal risk factors in the population : prognosis , prevalence , and secular trends ; data from Gteborg population studies .
	manualset3
123926	1	404329	13	NULL	NULL	0	NULL	Optimal treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal treatment consists of surgery followed by combination chemotherapy .
	manualset3
123927	2	404329	13	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal treatment consists of surgery followed by combination chemotherapy .
	manualset3
123928	3	404329	13	NULL	NULL	0	NULL	combination chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimal treatment consists of surgery followed by combination chemotherapy .
	manualset3
123930	1	404330	13	NULL	NULL	NULL	NULL	disintegrin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A disintegrin and metalloproteinase with thrombospondin motifs ( ADAMTS ) is a group of multifunctional proteinases .
	manualset3
123931	2	404330	13	NULL	NULL	0	NULL	metalloproteinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A disintegrin and metalloproteinase with thrombospondin motifs ( ADAMTS ) is a group of multifunctional proteinases .
	manualset3
123932	3	404330	13	NULL	NULL	0	NULL	thrombospondin motifs ( ADAMTS ) 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A disintegrin and metalloproteinase with thrombospondin motifs ( ADAMTS ) is a group of multifunctional proteinases .
	manualset3
123933	4	404330	13	NULL	NULL	0	NULL	group of multifunctional proteinases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A disintegrin and metalloproteinase with thrombospondin motifs ( ADAMTS ) is a group of multifunctional proteinases .
	manualset3
123939	1	404331	13	NULL	NULL	0	NULL	Optimisation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimisation of cosolvent concentration for topical drug delivery III -- influence of lipophilic vehicles on ibuprofen permeation .
	manualset3
123940	2	404331	13	NULL	NULL	0	NULL	cosolvent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimisation of cosolvent concentration for topical drug delivery III -- influence of lipophilic vehicles on ibuprofen permeation .
	manualset3
123941	3	404331	13	NULL	NULL	0	NULL	concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimisation of cosolvent concentration for topical drug delivery III -- influence of lipophilic vehicles on ibuprofen permeation .
	manualset3
123944	4	404331	13	NULL	NULL	0	NULL	topical drug delivery III	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimisation of cosolvent concentration for topical drug delivery III -- influence of lipophilic vehicles on ibuprofen permeation .
	manualset3
123945	5	404331	13	NULL	NULL	0	NULL	influence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimisation of cosolvent concentration for topical drug delivery III -- influence of lipophilic vehicles on ibuprofen permeation .
	manualset3
123946	6	404331	13	NULL	NULL	0	NULL	lipophilic vehicles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimisation of cosolvent concentration for topical drug delivery III -- influence of lipophilic vehicles on ibuprofen permeation .
	manualset3
123947	7	404331	13	NULL	NULL	0	NULL	ibuprofen	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimisation of cosolvent concentration for topical drug delivery III -- influence of lipophilic vehicles on ibuprofen permeation .
	manualset3
123948	8	404331	13	NULL	NULL	0	NULL	permeation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimisation of cosolvent concentration for topical drug delivery III -- influence of lipophilic vehicles on ibuprofen permeation .
	manualset3
123949	1	404332	13	NULL	NULL	0	NULL	Optimization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimization of all these factors enables the preparation of monolithic structures in capillaries with inner diameters as low as 5 microm while retaining the desirable properties of monoliths prepared in much larger capillaries .
	manualset3
123950	2	404332	13	NULL	NULL	0	NULL	factors 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimization of all these factors enables the preparation of monolithic structures in capillaries with inner diameters as low as 5 microm while retaining the desirable properties of monoliths prepared in much larger capillaries .
	manualset3
123951	3	404332	13	NULL	NULL	0	NULL	preparation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimization of all these factors enables the preparation of monolithic structures in capillaries with inner diameters as low as 5 microm while retaining the desirable properties of monoliths prepared in much larger capillaries .
	manualset3
123952	4	404332	13	NULL	NULL	0	NULL	monolithic structures	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimization of all these factors enables the preparation of monolithic structures in capillaries with inner diameters as low as 5 microm while retaining the desirable properties of monoliths prepared in much larger capillaries .
	manualset3
123953	5	404332	13	NULL	NULL	0	NULL	capillaries	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimization of all these factors enables the preparation of monolithic structures in capillaries with inner diameters as low as 5 microm while retaining the desirable properties of monoliths prepared in much larger capillaries .
	manualset3
123954	6	404332	13	NULL	NULL	0	NULL	inner diameters	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimization of all these factors enables the preparation of monolithic structures in capillaries with inner diameters as low as 5 microm while retaining the desirable properties of monoliths prepared in much larger capillaries .
	manualset3
123955	7	404332	13	NULL	NULL	0	NULL	5 microm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimization of all these factors enables the preparation of monolithic structures in capillaries with inner diameters as low as 5 microm while retaining the desirable properties of monoliths prepared in much larger capillaries .
	manualset3
123956	8	404332	13	NULL	NULL	0	NULL	desirable properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimization of all these factors enables the preparation of monolithic structures in capillaries with inner diameters as low as 5 microm while retaining the desirable properties of monoliths prepared in much larger capillaries .
	manualset3
123957	9	404332	13	NULL	NULL	0	NULL	monoliths	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimization of all these factors enables the preparation of monolithic structures in capillaries with inner diameters as low as 5 microm while retaining the desirable properties of monoliths prepared in much larger capillaries .
	manualset3
123958	10	404332	13	NULL	NULL	0	NULL	capillaries 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimization of all these factors enables the preparation of monolithic structures in capillaries with inner diameters as low as 5 microm while retaining the desirable properties of monoliths prepared in much larger capillaries .
	manualset3
123959	1	404333	13	NULL	NULL	0	NULL	Optimization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimization of levofloxacin analysis was carried out using multivariate calibration technique and detector response was recorded at five different wave lengths .
	manualset3
123960	2	404333	13	NULL	NULL	0	NULL	levofloxacin analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimization of levofloxacin analysis was carried out using multivariate calibration technique and detector response was recorded at five different wave lengths .
	manualset3
123961	3	404333	13	NULL	NULL	0	NULL	multivariate calibration technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimization of levofloxacin analysis was carried out using multivariate calibration technique and detector response was recorded at five different wave lengths .
	manualset3
123962	4	404333	13	NULL	NULL	0	NULL	detector response 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimization of levofloxacin analysis was carried out using multivariate calibration technique and detector response was recorded at five different wave lengths .
	manualset3
123963	5	404333	13	NULL	NULL	0	NULL	five	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimization of levofloxacin analysis was carried out using multivariate calibration technique and detector response was recorded at five different wave lengths .
	manualset3
123964	6	404333	13	NULL	NULL	0	NULL	wave lengths	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimization of levofloxacin analysis was carried out using multivariate calibration technique and detector response was recorded at five different wave lengths .
	manualset3
123965	1	404334	13	NULL	NULL	0	NULL	Phytoplasma DNA purification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimizing Phytoplasma DNA purification for genome analysis .
	manualset3
123966	2	404334	13	NULL	NULL	0	NULL	genome analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimizing Phytoplasma DNA purification for genome analysis .
	manualset3
123967	1	404335	13	NULL	NULL	NULL	NULL	analysis pipelines	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Optimizing preprocessing and analysis pipelines for single-subject fMRI .
	manualset3
123968	2	404335	13	NULL	NULL	NULL	NULL	 single-subject fMRI	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Optimizing preprocessing and analysis pipelines for single-subject fMRI .
	manualset3
125244	3	404335	13	NULL	NULL	0	NULL	preprocessing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimizing preprocessing and analysis pipelines for single-subject fMRI .
	manualset3
123969	1	404336	13	NULL	NULL	0	NULL	allocation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimum allocation of conservation funds and choice of conservation programs for a set of African cattle breeds .
	manualset3
123970	2	404336	13	NULL	NULL	0	NULL	conservation funds	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimum allocation of conservation funds and choice of conservation programs for a set of African cattle breeds .
	manualset3
123971	3	404336	13	NULL	NULL	0	NULL	choice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimum allocation of conservation funds and choice of conservation programs for a set of African cattle breeds .
	manualset3
123972	4	404336	13	NULL	NULL	0	NULL	conservation programs	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimum allocation of conservation funds and choice of conservation programs for a set of African cattle breeds .
	manualset3
123973	5	404336	13	NULL	NULL	0	NULL	set of African cattle breeds 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimum allocation of conservation funds and choice of conservation programs for a set of African cattle breeds .
	manualset3
123974	1	404337	13	NULL	NULL	0	NULL	Optimum conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimum conditions for GLC analysis of neomycin .
	manualset3
123975	2	404337	13	NULL	NULL	0	NULL	GLC analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimum conditions for GLC analysis of neomycin .
	manualset3
123976	3	404337	13	NULL	NULL	0	NULL	neomycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimum conditions for GLC analysis of neomycin .
	manualset3
123977	1	404338	13	NULL	NULL	0	NULL	Optimum configuration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimum configuration of cannulated hip screws for the fixation of intracapsular hip fractures : a biomechanical study .
	manualset3
123978	2	404338	13	NULL	NULL	0	NULL	hip screws	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimum configuration of cannulated hip screws for the fixation of intracapsular hip fractures : a biomechanical study .
	manualset3
123979	3	404338	13	NULL	NULL	0	NULL	fixation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimum configuration of cannulated hip screws for the fixation of intracapsular hip fractures : a biomechanical study .
	manualset3
123980	4	404338	13	NULL	NULL	0	NULL	intracapsular hip fractures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimum configuration of cannulated hip screws for the fixation of intracapsular hip fractures : a biomechanical study .
	manualset3
123981	5	404338	13	NULL	NULL	0	NULL	biomechanical study	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimum configuration of cannulated hip screws for the fixation of intracapsular hip fractures : a biomechanical study .
	manualset3
123982	1	404339	13	NULL	NULL	0	NULL	Optimum degree	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimum degree of maturity was also tested by germination index ( GI ) .
	manualset3
123983	2	404339	13	NULL	NULL	0	NULL	maturity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimum degree of maturity was also tested by germination index ( GI ) .
	manualset3
123984	3	404339	13	NULL	NULL	0	NULL	germination index ( GI )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimum degree of maturity was also tested by germination index ( GI ) .
	manualset3
123985	1	404340	13	NULL	NULL	0	NULL	disorder 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A disorder of the endogenous opioid peptide system ?
	manualset3
123986	2	404340	13	NULL	NULL	0	NULL	endogenous opioid peptide system 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A disorder of the endogenous opioid peptide system ?
	manualset3
123987	1	404341	13	NULL	NULL	0	NULL	Options	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Options for disposal are limited .
	manualset3
123988	2	404341	13	NULL	NULL	0	NULL	disposal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Options for disposal are limited .
	manualset3
123989	1	404342	13	NULL	NULL	0	NULL	Options	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Options for the treatment of pregnant women with obstructing stones include ureteral stent placement , percutaneous nephrostomy tube placement , and ureteroscopic stone removal ( URS ) .
	manualset3
123990	2	404342	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Options for the treatment of pregnant women with obstructing stones include ureteral stent placement , percutaneous nephrostomy tube placement , and ureteroscopic stone removal ( URS ) .
	manualset3
123991	3	404342	13	NULL	NULL	0	NULL	pregnant women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Options for the treatment of pregnant women with obstructing stones include ureteral stent placement , percutaneous nephrostomy tube placement , and ureteroscopic stone removal ( URS ) .
	manualset3
123992	4	404342	13	NULL	NULL	0	NULL	stones 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Options for the treatment of pregnant women with obstructing stones include ureteral stent placement , percutaneous nephrostomy tube placement , and ureteroscopic stone removal ( URS ) .
	manualset3
123993	5	404342	13	NULL	NULL	0	NULL	ureteral stent placement	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Options for the treatment of pregnant women with obstructing stones include ureteral stent placement , percutaneous nephrostomy tube placement , and ureteroscopic stone removal ( URS ) .
	manualset3
123994	6	404342	13	NULL	NULL	0	NULL	percutaneous nephrostomy tube placement	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Options for the treatment of pregnant women with obstructing stones include ureteral stent placement , percutaneous nephrostomy tube placement , and ureteroscopic stone removal ( URS ) .
	manualset3
123995	7	404342	13	NULL	NULL	0	NULL	ureteroscopic stone removal ( URS )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Options for the treatment of pregnant women with obstructing stones include ureteral stent placement , percutaneous nephrostomy tube placement , and ureteroscopic stone removal ( URS ) .
	manualset3
123996	1	404343	13	NULL	NULL	0	NULL	Oral administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral administration of 2-docosahexaenoyl lysophosphatidylcholine displayed anti-inflammatory effects on zymosan A-induced peritonitis .
	manualset3
123997	2	404343	13	NULL	NULL	0	NULL	2-docosahexaenoyl lysophosphatidylcholine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral administration of 2-docosahexaenoyl lysophosphatidylcholine displayed anti-inflammatory effects on zymosan A-induced peritonitis .
	manualset3
123998	3	404343	13	NULL	NULL	0	NULL	anti-inflammatory effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral administration of 2-docosahexaenoyl lysophosphatidylcholine displayed anti-inflammatory effects on zymosan A-induced peritonitis .
	manualset3
123999	4	404343	13	NULL	NULL	0	NULL	zymosan A-induced peritonitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral administration of 2-docosahexaenoyl lysophosphatidylcholine displayed anti-inflammatory effects on zymosan A-induced peritonitis .
	manualset3
124000	1	404344	13	NULL	NULL	0	NULL	Oral administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral administration of various anthraquinone components results in a rise in their blood concentrations , wide systemic distribution , accumulation in the liver and kidneys , and excretion in urine and feces ; polysaccharide components are distributed systemically and metabolized into smaller molecules .
	manualset3
124001	2	404344	13	NULL	NULL	0	NULL	various anthraquinone components 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral administration of various anthraquinone components results in a rise in their blood concentrations , wide systemic distribution , accumulation in the liver and kidneys , and excretion in urine and feces ; polysaccharide components are distributed systemically and metabolized into smaller molecules .
	manualset3
124002	3	404344	13	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral administration of various anthraquinone components results in a rise in their blood concentrations , wide systemic distribution , accumulation in the liver and kidneys , and excretion in urine and feces ; polysaccharide components are distributed systemically and metabolized into smaller molecules .
	manualset3
124003	4	404344	13	NULL	NULL	0	NULL	rise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral administration of various anthraquinone components results in a rise in their blood concentrations , wide systemic distribution , accumulation in the liver and kidneys , and excretion in urine and feces ; polysaccharide components are distributed systemically and metabolized into smaller molecules .
	manualset3
124004	5	404344	13	NULL	NULL	0	NULL	blood concentrations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral administration of various anthraquinone components results in a rise in their blood concentrations , wide systemic distribution , accumulation in the liver and kidneys , and excretion in urine and feces ; polysaccharide components are distributed systemically and metabolized into smaller molecules .
	manualset3
124005	6	404344	13	NULL	NULL	0	NULL	wide systemic distribution	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral administration of various anthraquinone components results in a rise in their blood concentrations , wide systemic distribution , accumulation in the liver and kidneys , and excretion in urine and feces ; polysaccharide components are distributed systemically and metabolized into smaller molecules .
	manualset3
124006	7	404344	13	NULL	NULL	0	NULL	accumulation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral administration of various anthraquinone components results in a rise in their blood concentrations , wide systemic distribution , accumulation in the liver and kidneys , and excretion in urine and feces ; polysaccharide components are distributed systemically and metabolized into smaller molecules .
	manualset3
124007	8	404344	13	NULL	NULL	0	NULL	liver 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral administration of various anthraquinone components results in a rise in their blood concentrations , wide systemic distribution , accumulation in the liver and kidneys , and excretion in urine and feces ; polysaccharide components are distributed systemically and metabolized into smaller molecules .
	manualset3
124008	9	404344	13	NULL	NULL	0	NULL	kidneys	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral administration of various anthraquinone components results in a rise in their blood concentrations , wide systemic distribution , accumulation in the liver and kidneys , and excretion in urine and feces ; polysaccharide components are distributed systemically and metabolized into smaller molecules .
	manualset3
124009	10	404344	13	NULL	NULL	0	NULL	excretion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral administration of various anthraquinone components results in a rise in their blood concentrations , wide systemic distribution , accumulation in the liver and kidneys , and excretion in urine and feces ; polysaccharide components are distributed systemically and metabolized into smaller molecules .
	manualset3
124010	11	404344	13	NULL	NULL	0	NULL	urine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral administration of various anthraquinone components results in a rise in their blood concentrations , wide systemic distribution , accumulation in the liver and kidneys , and excretion in urine and feces ; polysaccharide components are distributed systemically and metabolized into smaller molecules .
	manualset3
124011	12	404344	13	NULL	NULL	0	NULL	feces	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral administration of various anthraquinone components results in a rise in their blood concentrations , wide systemic distribution , accumulation in the liver and kidneys , and excretion in urine and feces ; polysaccharide components are distributed systemically and metabolized into smaller molecules .
	manualset3
124012	13	404344	13	NULL	NULL	0	NULL	polysaccharide components	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral administration of various anthraquinone components results in a rise in their blood concentrations , wide systemic distribution , accumulation in the liver and kidneys , and excretion in urine and feces ; polysaccharide components are distributed systemically and metabolized into smaller molecules .
	manualset3
124013	14	404344	13	NULL	NULL	0	NULL	smaller molecules	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral administration of various anthraquinone components results in a rise in their blood concentrations , wide systemic distribution , accumulation in the liver and kidneys , and excretion in urine and feces ; polysaccharide components are distributed systemically and metabolized into smaller molecules .
	manualset3
124014	1	404345	13	NULL	NULL	0	NULL	flecainide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral flecainide is , therefore , subject to the same problems of varying oral bioavailability as other antiarrhythmic drugs tested following acute myocardial infarction and , initially , an intravenous regime remains preferable .
	manualset3
124015	2	404345	13	NULL	NULL	0	NULL	problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral flecainide is , therefore , subject to the same problems of varying oral bioavailability as other antiarrhythmic drugs tested following acute myocardial infarction and , initially , an intravenous regime remains preferable .
	manualset3
124016	3	404345	13	NULL	NULL	0	NULL	oral bioavailability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral flecainide is , therefore , subject to the same problems of varying oral bioavailability as other antiarrhythmic drugs tested following acute myocardial infarction and , initially , an intravenous regime remains preferable .
	manualset3
124017	4	404345	13	NULL	NULL	0	NULL	antiarrhythmic drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral flecainide is , therefore , subject to the same problems of varying oral bioavailability as other antiarrhythmic drugs tested following acute myocardial infarction and , initially , an intravenous regime remains preferable .
	manualset3
124018	5	404345	13	NULL	NULL	0	NULL	acute myocardial infarction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral flecainide is , therefore , subject to the same problems of varying oral bioavailability as other antiarrhythmic drugs tested following acute myocardial infarction and , initially , an intravenous regime remains preferable .
	manualset3
124019	6	404345	13	NULL	NULL	0	NULL	intravenous regime	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral flecainide is , therefore , subject to the same problems of varying oral bioavailability as other antiarrhythmic drugs tested following acute myocardial infarction and , initially , an intravenous regime remains preferable .
	manualset3
124020	1	404346	13	NULL	NULL	0	NULL	Oral fluids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral fluids were tested by GACELISA and corresponding serum samples by a sensitive indirect ELISA for measles IgG ( Behring Enzygnost ) .
	manualset3
124021	2	404346	13	NULL	NULL	0	NULL	GACELISA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral fluids were tested by GACELISA and corresponding serum samples by a sensitive indirect ELISA for measles IgG ( Behring Enzygnost ) .
	manualset3
124022	3	404346	13	NULL	NULL	0	NULL	serum samples 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral fluids were tested by GACELISA and corresponding serum samples by a sensitive indirect ELISA for measles IgG ( Behring Enzygnost ) .
	manualset3
124023	4	404346	13	NULL	NULL	0	NULL	ELISA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral fluids were tested by GACELISA and corresponding serum samples by a sensitive indirect ELISA for measles IgG ( Behring Enzygnost ) .
	manualset3
124024	5	404346	13	NULL	NULL	0	NULL	measles IgG 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral fluids were tested by GACELISA and corresponding serum samples by a sensitive indirect ELISA for measles IgG ( Behring Enzygnost ) .
	manualset3
124025	6	404346	13	NULL	NULL	0	NULL	Behring Enzygnost	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral fluids were tested by GACELISA and corresponding serum samples by a sensitive indirect ELISA for measles IgG ( Behring Enzygnost ) .
	manualset3
124026	1	404347	13	NULL	NULL	0	NULL	dispersive model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A dispersive model for the propagation of ultrasound in soft tissue .
	manualset3
124027	2	404347	13	NULL	NULL	0	NULL	propagation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A dispersive model for the propagation of ultrasound in soft tissue .
	manualset3
124028	3	404347	13	NULL	NULL	0	NULL	ultrasound	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A dispersive model for the propagation of ultrasound in soft tissue .
	manualset3
124029	4	404347	13	NULL	NULL	0	NULL	soft tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	A dispersive model for the propagation of ultrasound in soft tissue .
	manualset3
124030	1	404348	13	NULL	NULL	0	NULL	Oral immunization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral immunization of rabbits with VP60 particles confers protection against rabbit hemorrhagic disease .
	manualset3
124031	2	404348	13	NULL	NULL	0	NULL	rabbits 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral immunization of rabbits with VP60 particles confers protection against rabbit hemorrhagic disease .
	manualset3
124032	3	404348	13	NULL	NULL	0	NULL	VP60 particles	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral immunization of rabbits with VP60 particles confers protection against rabbit hemorrhagic disease .
	manualset3
124033	4	404348	13	NULL	NULL	0	NULL	protection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral immunization of rabbits with VP60 particles confers protection against rabbit hemorrhagic disease .
	manualset3
124034	5	404348	13	NULL	NULL	0	NULL	rabbit hemorrhagic disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral immunization of rabbits with VP60 particles confers protection against rabbit hemorrhagic disease .
	manualset3
124035	1	404349	13	NULL	NULL	0	NULL	Oral lichen planus ( OLP ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral lichen planus ( OLP ) , one of the most common oral mucosa diseases , is an auto-immune disease characterized histologically by basal keratinocyte damage and interface lymphocyte reaction .
	manualset3
124036	2	404349	13	NULL	NULL	0	NULL	oral mucosa diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral lichen planus ( OLP ) , one of the most common oral mucosa diseases , is an auto-immune disease characterized histologically by basal keratinocyte damage and interface lymphocyte reaction .
	manualset3
124037	3	404349	13	NULL	NULL	0	NULL	auto-immune disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral lichen planus ( OLP ) , one of the most common oral mucosa diseases , is an auto-immune disease characterized histologically by basal keratinocyte damage and interface lymphocyte reaction .
	manualset3
124038	4	404349	13	NULL	NULL	0	NULL	basal keratinocyte damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral lichen planus ( OLP ) , one of the most common oral mucosa diseases , is an auto-immune disease characterized histologically by basal keratinocyte damage and interface lymphocyte reaction .
	manualset3
124039	5	404349	13	NULL	NULL	0	NULL	interface lymphocyte reaction 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral lichen planus ( OLP ) , one of the most common oral mucosa diseases , is an auto-immune disease characterized histologically by basal keratinocyte damage and interface lymphocyte reaction .
	manualset3
124040	1	404350	13	NULL	NULL	0	NULL	Oral malodorous compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral malodorous compound causes apoptosis and genomic DNA damage in human gingival fibroblasts .
	manualset3
124041	2	404350	13	NULL	NULL	0	NULL	apoptosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral malodorous compound causes apoptosis and genomic DNA damage in human gingival fibroblasts .
	manualset3
124042	3	404350	13	NULL	NULL	0	NULL	genomic DNA damage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral malodorous compound causes apoptosis and genomic DNA damage in human gingival fibroblasts .
	manualset3
124043	4	404350	13	NULL	NULL	0	NULL	human gingival fibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral malodorous compound causes apoptosis and genomic DNA damage in human gingival fibroblasts .
	manualset3
124044	1	404351	13	NULL	NULL	0	NULL	Oral olive oil	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral olive oil , 4 ml/kg , was used as control .
	manualset3
124045	2	404351	13	NULL	NULL	0	NULL	4 ml/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral olive oil , 4 ml/kg , was used as control .
	manualset3
124046	3	404351	13	NULL	NULL	0	NULL	control 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral olive oil , 4 ml/kg , was used as control .
	manualset3
124047	1	404352	13	NULL	NULL	0	NULL	Oral precancerous lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral precancerous lesions : a review .
	manualset3
124048	2	404352	13	NULL	NULL	0	NULL	review	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral precancerous lesions : a review .
	manualset3
124049	1	404353	13	NULL	NULL	0	NULL	Oral transmission	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral transmission of BSE to VRQ/VRQ sheep in an experimental flock .
	manualset3
124050	2	404353	13	NULL	NULL	0	NULL	BSE	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral transmission of BSE to VRQ/VRQ sheep in an experimental flock .
	manualset3
124051	3	404353	13	NULL	NULL	0	NULL	VRQ/VRQ sheep	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral transmission of BSE to VRQ/VRQ sheep in an experimental flock .
	manualset3
124052	4	404353	13	NULL	NULL	0	NULL	experimental flock	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral transmission of BSE to VRQ/VRQ sheep in an experimental flock .
	manualset3
124053	1	404354	13	NULL	NULL	0	NULL	Oral treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral treatment was started with oral aciclovir and corticosteroids for 2 months , when she had resolution of the optic neuropathy and ophthalmoplegia .
	manualset3
124054	2	404354	13	NULL	NULL	0	NULL	oral aciclovir	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral treatment was started with oral aciclovir and corticosteroids for 2 months , when she had resolution of the optic neuropathy and ophthalmoplegia .
	manualset3
124055	3	404354	13	NULL	NULL	0	NULL	corticosteroids	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral treatment was started with oral aciclovir and corticosteroids for 2 months , when she had resolution of the optic neuropathy and ophthalmoplegia .
	manualset3
124056	4	404354	13	NULL	NULL	0	NULL	2 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral treatment was started with oral aciclovir and corticosteroids for 2 months , when she had resolution of the optic neuropathy and ophthalmoplegia .
	manualset3
124057	5	404354	13	NULL	NULL	0	NULL	resolution	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral treatment was started with oral aciclovir and corticosteroids for 2 months , when she had resolution of the optic neuropathy and ophthalmoplegia .
	manualset3
124058	6	404354	13	NULL	NULL	0	NULL	optic neuropathy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral treatment was started with oral aciclovir and corticosteroids for 2 months , when she had resolution of the optic neuropathy and ophthalmoplegia .
	manualset3
124059	7	404354	13	NULL	NULL	0	NULL	ophthalmoplegia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral treatment was started with oral aciclovir and corticosteroids for 2 months , when she had resolution of the optic neuropathy and ophthalmoplegia .
	manualset3
124060	1	404355	13	NULL	NULL	NULL	NULL	zinc sulphate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Oral zinc sulphate treatment of chronic non-sickle cell ulcers in Jamaica .
	manualset3
124061	2	404355	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral zinc sulphate treatment of chronic non-sickle cell ulcers in Jamaica .
	manualset3
124062	3	404355	13	NULL	NULL	0	NULL	chronic non-sickle cell ulcers	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral zinc sulphate treatment of chronic non-sickle cell ulcers in Jamaica .
	manualset3
124063	4	404355	13	NULL	NULL	0	NULL	Jamaica	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral zinc sulphate treatment of chronic non-sickle cell ulcers in Jamaica .
	manualset3
124064	1	404356	13	NULL	NULL	0	NULL	Orbital implants 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Orbital implants after enucleation ; causes of complications and their solution .
	manualset3
124065	2	404356	13	NULL	NULL	0	NULL	enucleation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Orbital implants after enucleation ; causes of complications and their solution .
	manualset3
124066	3	404356	13	NULL	NULL	0	NULL	causes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Orbital implants after enucleation ; causes of complications and their solution .
	manualset3
124067	4	404356	13	NULL	NULL	0	NULL	complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Orbital implants after enucleation ; causes of complications and their solution .
	manualset3
124068	5	404356	13	NULL	NULL	0	NULL	solution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Orbital implants after enucleation ; causes of complications and their solution .
	manualset3
124069	1	404357	13	NULL	NULL	0	NULL	transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ordered transcription of RNA tumor virus genomes .
	manualset3
124070	2	404357	13	NULL	NULL	0	NULL	RNA tumor virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ordered transcription of RNA tumor virus genomes .
	manualset3
124071	3	404357	13	NULL	NULL	0	NULL	genomes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Ordered transcription of RNA tumor virus genomes .
	manualset3
124072	1	404358	13	NULL	NULL	0	NULL	Organization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Organization and regulation of collagen genes .
	manualset3
124073	2	404358	13	NULL	NULL	0	NULL	regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Organization and regulation of collagen genes .
	manualset3
124074	3	404358	13	NULL	NULL	0	NULL	collagen genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Organization and regulation of collagen genes .
	manualset3
124075	1	404359	13	NULL	NULL	0	NULL	Organogelators	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Organo - and hydrogelators based on luminescent monocationic terpyridyl platinum ( II ) complexes with biphenylacetylide ligands .
	manualset3
124076	2	404359	13	NULL	NULL	0	NULL	hydrogelators	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Organo - and hydrogelators based on luminescent monocationic terpyridyl platinum ( II ) complexes with biphenylacetylide ligands .
	manualset3
124077	3	404359	13	NULL	NULL	0	NULL	luminescent monocationic terpyridyl platinum ( II ) complexes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Organo - and hydrogelators based on luminescent monocationic terpyridyl platinum ( II ) complexes with biphenylacetylide ligands .
	manualset3
124078	4	404359	13	NULL	NULL	0	NULL	biphenylacetylide ligands 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Organo - and hydrogelators based on luminescent monocationic terpyridyl platinum ( II ) complexes with biphenylacetylide ligands .
	manualset3
124079	1	404360	13	NULL	NULL	0	NULL	Organometallic electrodes	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Organometallic electrodes : modification of electrode surfaces through cathodic reduction of cyclopentadienyldiazonium complexes of cobalt and manganese .
	manualset3
124080	2	404360	13	NULL	NULL	0	NULL	modification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Organometallic electrodes : modification of electrode surfaces through cathodic reduction of cyclopentadienyldiazonium complexes of cobalt and manganese .
	manualset3
124081	3	404360	13	NULL	NULL	0	NULL	electrode surfaces 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Organometallic electrodes : modification of electrode surfaces through cathodic reduction of cyclopentadienyldiazonium complexes of cobalt and manganese .
	manualset3
124082	4	404360	13	NULL	NULL	0	NULL	cathodic reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Organometallic electrodes : modification of electrode surfaces through cathodic reduction of cyclopentadienyldiazonium complexes of cobalt and manganese .
	manualset3
124083	5	404360	13	NULL	NULL	0	NULL	cyclopentadienyldiazonium complexes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Organometallic electrodes : modification of electrode surfaces through cathodic reduction of cyclopentadienyldiazonium complexes of cobalt and manganese .
	manualset3
124084	6	404360	13	NULL	NULL	0	NULL	cobalt	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Organometallic electrodes : modification of electrode surfaces through cathodic reduction of cyclopentadienyldiazonium complexes of cobalt and manganese .
	manualset3
124085	7	404360	13	NULL	NULL	0	NULL	manganese	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Organometallic electrodes : modification of electrode surfaces through cathodic reduction of cyclopentadienyldiazonium complexes of cobalt and manganese .
	manualset3
124086	1	404361	13	NULL	NULL	0	NULL	Organotrophic growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Organotrophic growth occurred on complex organic substrates such as yeast extract and peptone and on organic acids .
	manualset3
124087	2	404361	13	NULL	NULL	0	NULL	complex organic substrates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Organotrophic growth occurred on complex organic substrates such as yeast extract and peptone and on organic acids .
	manualset3
124088	3	404361	13	NULL	NULL	0	NULL	yeast extract	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Organotrophic growth occurred on complex organic substrates such as yeast extract and peptone and on organic acids .
	manualset3
124089	4	404361	13	NULL	NULL	0	NULL	peptone	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Organotrophic growth occurred on complex organic substrates such as yeast extract and peptone and on organic acids .
	manualset3
124090	5	404361	13	NULL	NULL	0	NULL	organic acids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Organotrophic growth occurred on complex organic substrates such as yeast extract and peptone and on organic acids .
	manualset3
124091	1	404362	13	NULL	NULL	0	NULL	Origin	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Origin of p-aminobenzoic acid from chorismic rather than iso-chorismic acid in Enterobacter aerogenes and Streptomyces species .
	manualset3
124092	2	404362	13	NULL	NULL	0	NULL	p-aminobenzoic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Origin of p-aminobenzoic acid from chorismic rather than iso-chorismic acid in Enterobacter aerogenes and Streptomyces species .
	manualset3
124094	3	404362	13	NULL	NULL	0	NULL	chorismic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Origin of p-aminobenzoic acid from chorismic rather than iso-chorismic acid in Enterobacter aerogenes and Streptomyces species .
	manualset3
124095	4	404362	13	NULL	NULL	0	NULL	iso-chorismic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Origin of p-aminobenzoic acid from chorismic rather than iso-chorismic acid in Enterobacter aerogenes and Streptomyces species .
	manualset3
124096	5	404362	13	NULL	NULL	0	NULL	Enterobacter aerogenes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Origin of p-aminobenzoic acid from chorismic rather than iso-chorismic acid in Enterobacter aerogenes and Streptomyces species .
	manualset3
124097	6	404362	13	NULL	NULL	0	NULL	Streptomyces species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Origin of p-aminobenzoic acid from chorismic rather than iso-chorismic acid in Enterobacter aerogenes and Streptomyces species .
	manualset3
124098	1	404363	13	NULL	NULL	0	NULL	2011	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	( 2011 ) Influenza transmission during a one-year period ( 2009-2010 ) in a Sahelian city : low temperature plays a major role .
	manualset3
124099	2	404363	13	NULL	NULL	0	NULL	Influenza transmission	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( 2011 ) Influenza transmission during a one-year period ( 2009-2010 ) in a Sahelian city : low temperature plays a major role .
	manualset3
124100	3	404363	13	NULL	NULL	0	NULL	one-year period ( 2009-2010 )	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	( 2011 ) Influenza transmission during a one-year period ( 2009-2010 ) in a Sahelian city : low temperature plays a major role .
	manualset3
124101	4	404363	13	NULL	NULL	0	NULL	Sahelian city	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( 2011 ) Influenza transmission during a one-year period ( 2009-2010 ) in a Sahelian city : low temperature plays a major role .
	manualset3
124102	5	404363	13	NULL	NULL	0	NULL	low temperature	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( 2011 ) Influenza transmission during a one-year period ( 2009-2010 ) in a Sahelian city : low temperature plays a major role .
	manualset3
124103	6	404363	13	NULL	NULL	0	NULL	role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( 2011 ) Influenza transmission during a one-year period ( 2009-2010 ) in a Sahelian city : low temperature plays a major role .
	manualset3
124104	1	404364	13	NULL	NULL	0	NULL	Bone marrow biopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Bone marrow biopsy in non-Hodgkin 's lymphoma : experience with 259 samples ) .
	manualset3
124105	2	404364	13	NULL	NULL	0	NULL	non-Hodgkin 's lymphoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Bone marrow biopsy in non-Hodgkin 's lymphoma : experience with 259 samples ) .
	manualset3
124106	3	404364	13	NULL	NULL	0	NULL	experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Bone marrow biopsy in non-Hodgkin 's lymphoma : experience with 259 samples ) .
	manualset3
124107	4	404364	13	NULL	NULL	0	NULL	 259 samples 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( Bone marrow biopsy in non-Hodgkin 's lymphoma : experience with 259 samples ) .
	manualset3
124108	1	404365	13	NULL	NULL	0	NULL	heteromorphism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A distinct heteromorphism in banding pattern was detected on the long arm of chromosome 9 in these embryos , but the frequency of this variant was too low for chromosome 9 to be a sex chromosome .
	manualset3
124109	2	404365	13	NULL	NULL	0	NULL	pattern	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A distinct heteromorphism in banding pattern was detected on the long arm of chromosome 9 in these embryos , but the frequency of this variant was too low for chromosome 9 to be a sex chromosome .
	manualset3
124110	3	404365	13	NULL	NULL	0	NULL	long arm	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	A distinct heteromorphism in banding pattern was detected on the long arm of chromosome 9 in these embryos , but the frequency of this variant was too low for chromosome 9 to be a sex chromosome .
	manualset3
124111	4	404365	13	NULL	NULL	0	NULL	chromosome 9 	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	A distinct heteromorphism in banding pattern was detected on the long arm of chromosome 9 in these embryos , but the frequency of this variant was too low for chromosome 9 to be a sex chromosome .
	manualset3
124112	5	404365	13	NULL	NULL	0	NULL	embryos	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A distinct heteromorphism in banding pattern was detected on the long arm of chromosome 9 in these embryos , but the frequency of this variant was too low for chromosome 9 to be a sex chromosome .
	manualset3
124113	6	404365	13	NULL	NULL	0	NULL	frequency	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A distinct heteromorphism in banding pattern was detected on the long arm of chromosome 9 in these embryos , but the frequency of this variant was too low for chromosome 9 to be a sex chromosome .
	manualset3
124114	7	404365	13	NULL	NULL	0	NULL	variant	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	A distinct heteromorphism in banding pattern was detected on the long arm of chromosome 9 in these embryos , but the frequency of this variant was too low for chromosome 9 to be a sex chromosome .
	manualset3
124115	8	404365	13	NULL	NULL	0	NULL	chromosome 9	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	A distinct heteromorphism in banding pattern was detected on the long arm of chromosome 9 in these embryos , but the frequency of this variant was too low for chromosome 9 to be a sex chromosome .
	manualset3
124116	9	404365	13	NULL	NULL	0	NULL	sex chromosome	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	A distinct heteromorphism in banding pattern was detected on the long arm of chromosome 9 in these embryos , but the frequency of this variant was too low for chromosome 9 to be a sex chromosome .
	manualset3
124117	1	404366	13	NULL	NULL	0	NULL	Origins of lateral hypothalamic afferents	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Origins of lateral hypothalamic afferents associated with N-methyl-d-aspartic acid-elicited eating studied using reverse microdialysis of NMDA and Fluorogold .
	manualset3
124118	2	404366	13	NULL	NULL	0	NULL	N-methyl-d-aspartic acid-elicited eating	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Origins of lateral hypothalamic afferents associated with N-methyl-d-aspartic acid-elicited eating studied using reverse microdialysis of NMDA and Fluorogold .
	manualset3
124119	3	404366	13	NULL	NULL	NULL	NULL	reverse microdialysis	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Origins of lateral hypothalamic afferents associated with N-methyl-d-aspartic acid-elicited eating studied using reverse microdialysis of NMDA and Fluorogold .
	manualset3
124120	4	404366	13	NULL	NULL	0	NULL	 NMDA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Origins of lateral hypothalamic afferents associated with N-methyl-d-aspartic acid-elicited eating studied using reverse microdialysis of NMDA and Fluorogold .
	manualset3
124121	5	404366	13	NULL	NULL	0	NULL	Fluorogold 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Origins of lateral hypothalamic afferents associated with N-methyl-d-aspartic acid-elicited eating studied using reverse microdialysis of NMDA and Fluorogold .
	manualset3
124122	1	404367	13	NULL	NULL	0	NULL	Ormocer 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ormocer : An aesthetic direct restorative material ; An in vitro study comparing the marginal sealing ability of organically modified ceramics and a hybrid composite using an ormocer-based bonding agent and a conventional fifth-generation bonding agent .
	manualset3
124123	2	404367	13	NULL	NULL	0	NULL	restorative material	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ormocer : An aesthetic direct restorative material ; An in vitro study comparing the marginal sealing ability of organically modified ceramics and a hybrid composite using an ormocer-based bonding agent and a conventional fifth-generation bonding agent .
	manualset3
124124	3	404367	13	NULL	NULL	0	NULL	in vitro study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ormocer : An aesthetic direct restorative material ; An in vitro study comparing the marginal sealing ability of organically modified ceramics and a hybrid composite using an ormocer-based bonding agent and a conventional fifth-generation bonding agent .
	manualset3
124125	4	404367	13	NULL	NULL	0	NULL	marginal sealing ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ormocer : An aesthetic direct restorative material ; An in vitro study comparing the marginal sealing ability of organically modified ceramics and a hybrid composite using an ormocer-based bonding agent and a conventional fifth-generation bonding agent .
	manualset3
124126	5	404367	13	NULL	NULL	0	NULL	ceramics 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Ormocer : An aesthetic direct restorative material ; An in vitro study comparing the marginal sealing ability of organically modified ceramics and a hybrid composite using an ormocer-based bonding agent and a conventional fifth-generation bonding agent .
	manualset3
124127	6	404367	13	NULL	NULL	0	NULL	agent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ormocer : An aesthetic direct restorative material ; An in vitro study comparing the marginal sealing ability of organically modified ceramics and a hybrid composite using an ormocer-based bonding agent and a conventional fifth-generation bonding agent .
	manualset3
124128	7	404367	13	NULL	NULL	0	NULL	hybrid composite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ormocer : An aesthetic direct restorative material ; An in vitro study comparing the marginal sealing ability of organically modified ceramics and a hybrid composite using an ormocer-based bonding agent and a conventional fifth-generation bonding agent .
	manualset3
124129	8	404367	13	NULL	NULL	0	NULL	conventional fifth-generation bonding agent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ormocer : An aesthetic direct restorative material ; An in vitro study comparing the marginal sealing ability of organically modified ceramics and a hybrid composite using an ormocer-based bonding agent and a conventional fifth-generation bonding agent .
	manualset3
124130	1	404368	13	NULL	NULL	0	NULL	Ornithine decarboxylase ( ODC ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Ornithine decarboxylase ( ODC ) functions as a cell transition factor by regulating the biosynthesis of polyamines , which , allied with aberrant crypt foci ( ACF ) proliferation , cause early lesions of CRC .
	manualset3
124132	3	404368	13	NULL	NULL	0	NULL	cell transition factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Ornithine decarboxylase ( ODC ) functions as a cell transition factor by regulating the biosynthesis of polyamines , which , allied with aberrant crypt foci ( ACF ) proliferation , cause early lesions of CRC .
	manualset3
124133	4	404368	13	NULL	NULL	0	NULL	biosynthesis of polyamines	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ornithine decarboxylase ( ODC ) functions as a cell transition factor by regulating the biosynthesis of polyamines , which , allied with aberrant crypt foci ( ACF ) proliferation , cause early lesions of CRC .
	manualset3
124134	5	404368	13	NULL	NULL	0	NULL	aberrant crypt foci ( ACF ) proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ornithine decarboxylase ( ODC ) functions as a cell transition factor by regulating the biosynthesis of polyamines , which , allied with aberrant crypt foci ( ACF ) proliferation , cause early lesions of CRC .
	manualset3
124135	6	404368	13	NULL	NULL	0	NULL	lesions of CRC	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ornithine decarboxylase ( ODC ) functions as a cell transition factor by regulating the biosynthesis of polyamines , which , allied with aberrant crypt foci ( ACF ) proliferation , cause early lesions of CRC .
	manualset3
124136	1	404369	13	NULL	NULL	0	NULL	Orthologs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Orthologs of the Streptococcus iniae LysR family regulator CpsY have been shown to regulate methionine biosynthesis and uptake pathways but appear to influence expression of several virulence genes as well .
	manualset3
124137	2	404369	13	NULL	NULL	0	NULL	Streptococcus iniae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Orthologs of the Streptococcus iniae LysR family regulator CpsY have been shown to regulate methionine biosynthesis and uptake pathways but appear to influence expression of several virulence genes as well .
	manualset3
124138	3	404369	13	NULL	NULL	0	NULL	LysR family regulator	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Orthologs of the Streptococcus iniae LysR family regulator CpsY have been shown to regulate methionine biosynthesis and uptake pathways but appear to influence expression of several virulence genes as well .
	manualset3
124139	4	404369	13	NULL	NULL	0	NULL	CpsY	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Orthologs of the Streptococcus iniae LysR family regulator CpsY have been shown to regulate methionine biosynthesis and uptake pathways but appear to influence expression of several virulence genes as well .
	manualset3
124140	5	404369	13	NULL	NULL	0	NULL	methionine biosynthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Orthologs of the Streptococcus iniae LysR family regulator CpsY have been shown to regulate methionine biosynthesis and uptake pathways but appear to influence expression of several virulence genes as well .
	manualset3
124141	6	404369	13	NULL	NULL	0	NULL	uptake pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Orthologs of the Streptococcus iniae LysR family regulator CpsY have been shown to regulate methionine biosynthesis and uptake pathways but appear to influence expression of several virulence genes as well .
	manualset3
124143	8	404369	13	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Orthologs of the Streptococcus iniae LysR family regulator CpsY have been shown to regulate methionine biosynthesis and uptake pathways but appear to influence expression of several virulence genes as well .
	manualset3
124144	9	404369	13	NULL	NULL	0	NULL	several virulence genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Orthologs of the Streptococcus iniae LysR family regulator CpsY have been shown to regulate methionine biosynthesis and uptake pathways but appear to influence expression of several virulence genes as well .
	manualset3
124145	1	404370	13	NULL	NULL	0	NULL	Os odontoideum	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Os odontoideum : a significant radiographic finding .
	manualset3
124146	2	404370	13	NULL	NULL	0	NULL	radiographic finding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Os odontoideum : a significant radiographic finding .
	manualset3
124147	1	404371	13	NULL	NULL	0	NULL	Oscillatory changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Oscillatory changes in multiple unit activity during rapid eye movement sleep .
	manualset3
124148	2	404371	13	NULL	NULL	0	NULL	multiple unit activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Oscillatory changes in multiple unit activity during rapid eye movement sleep .
	manualset3
124149	3	404371	13	NULL	NULL	NULL	NULL	rapid eye movement sleep	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Oscillatory changes in multiple unit activity during rapid eye movement sleep .
	manualset3
124151	1	404372	13	NULL	NULL	0	NULL	Osmotic diuresis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Osmotic diuresis as treatment in severe hyponatremia .
	manualset3
124152	2	404372	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Osmotic diuresis as treatment in severe hyponatremia .
	manualset3
124153	3	404372	13	NULL	NULL	0	NULL	severe hyponatremia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Osmotic diuresis as treatment in severe hyponatremia .
	manualset3
124154	1	404373	13	NULL	NULL	0	NULL	Osmotic induction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Osmotic induction of rpoS can be triggered by addition of NaCl or sucrose and is alleviated by glycine betaine .
	manualset3
124155	2	404373	13	NULL	NULL	0	NULL	rpoS	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Osmotic induction of rpoS can be triggered by addition of NaCl or sucrose and is alleviated by glycine betaine .
	manualset3
124156	3	404373	13	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Osmotic induction of rpoS can be triggered by addition of NaCl or sucrose and is alleviated by glycine betaine .
	manualset3
124157	4	404373	13	NULL	NULL	0	NULL	NaCl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Osmotic induction of rpoS can be triggered by addition of NaCl or sucrose and is alleviated by glycine betaine .
	manualset3
124158	5	404373	13	NULL	NULL	0	NULL	sucrose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Osmotic induction of rpoS can be triggered by addition of NaCl or sucrose and is alleviated by glycine betaine .
	manualset3
124159	6	404373	13	NULL	NULL	0	NULL	glycine betaine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Osmotic induction of rpoS can be triggered by addition of NaCl or sucrose and is alleviated by glycine betaine .
	manualset3
124160	1	404374	13	NULL	NULL	NULL	NULL	Osmotic properties	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Osmotic properties of stallion sperm subpopulations determined by simultaneous assessment of cell volume and viability .
	manualset3
124161	2	404374	13	NULL	NULL	0	NULL	stallion sperm subpopulations	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Osmotic properties of stallion sperm subpopulations determined by simultaneous assessment of cell volume and viability .
	manualset3
124162	3	404374	13	NULL	NULL	0	NULL	 simultaneous assessment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Osmotic properties of stallion sperm subpopulations determined by simultaneous assessment of cell volume and viability .
	manualset3
124163	4	404374	13	NULL	NULL	0	NULL	cell volume 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Osmotic properties of stallion sperm subpopulations determined by simultaneous assessment of cell volume and viability .
	manualset3
124164	5	404374	13	NULL	NULL	0	NULL	viability	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Osmotic properties of stallion sperm subpopulations determined by simultaneous assessment of cell volume and viability .
	manualset3
124165	1	404375	13	NULL	NULL	0	NULL	distinction 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A distinction between stenosis and occlusion by UDS of the supratrochlear artery is , however , not possible , unless additional examination of the carotid arteries is performed .
	manualset3
124166	2	404375	13	NULL	NULL	0	NULL	stenosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A distinction between stenosis and occlusion by UDS of the supratrochlear artery is , however , not possible , unless additional examination of the carotid arteries is performed .
	manualset3
124167	3	404375	13	NULL	NULL	0	NULL	occlusion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A distinction between stenosis and occlusion by UDS of the supratrochlear artery is , however , not possible , unless additional examination of the carotid arteries is performed .
	manualset3
124168	4	404375	13	NULL	NULL	0	NULL	UDS	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A distinction between stenosis and occlusion by UDS of the supratrochlear artery is , however , not possible , unless additional examination of the carotid arteries is performed .
	manualset3
124169	5	404375	13	NULL	NULL	0	NULL	supratrochlear artery 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A distinction between stenosis and occlusion by UDS of the supratrochlear artery is , however , not possible , unless additional examination of the carotid arteries is performed .
	manualset3
124170	6	404375	13	NULL	NULL	0	NULL	examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A distinction between stenosis and occlusion by UDS of the supratrochlear artery is , however , not possible , unless additional examination of the carotid arteries is performed .
	manualset3
124171	7	404375	13	NULL	NULL	0	NULL	carotid arteries 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A distinction between stenosis and occlusion by UDS of the supratrochlear artery is , however , not possible , unless additional examination of the carotid arteries is performed .
	manualset3
124188	1	404376	13	NULL	NULL	0	NULL	Osteoarthralgia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Osteoarthralgia is a common symptom at the beginning of acute lymphoblastic leukemia ( ALL ) .
	manualset3
124189	2	404376	13	NULL	NULL	0	NULL	common symptom	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Osteoarthralgia is a common symptom at the beginning of acute lymphoblastic leukemia ( ALL ) .
	manualset3
124190	3	404376	13	NULL	NULL	0	NULL	beginning 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Osteoarthralgia is a common symptom at the beginning of acute lymphoblastic leukemia ( ALL ) .
	manualset3
124191	4	404376	13	NULL	NULL	0	NULL	acute lymphoblastic leukemia ( ALL )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Osteoarthralgia is a common symptom at the beginning of acute lymphoblastic leukemia ( ALL ) .
	manualset3
124192	1	404377	13	NULL	NULL	0	NULL	Osteoblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Osteoblasts on rod shaped hydroxyapatite nanoparticles incorporated PCL film provide an optimal osteogenic niche for stem cell differentiation .
	manualset3
124193	2	404377	13	NULL	NULL	0	NULL	rod shaped hydroxyapatite nanoparticles	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Osteoblasts on rod shaped hydroxyapatite nanoparticles incorporated PCL film provide an optimal osteogenic niche for stem cell differentiation .
	manualset3
124194	3	404377	13	NULL	NULL	0	NULL	PCL film	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Osteoblasts on rod shaped hydroxyapatite nanoparticles incorporated PCL film provide an optimal osteogenic niche for stem cell differentiation .
	manualset3
124195	4	404377	13	NULL	NULL	0	NULL	optimal osteogenic niche	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Osteoblasts on rod shaped hydroxyapatite nanoparticles incorporated PCL film provide an optimal osteogenic niche for stem cell differentiation .
	manualset3
124196	5	404377	13	NULL	NULL	0	NULL	stem cell differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Osteoblasts on rod shaped hydroxyapatite nanoparticles incorporated PCL film provide an optimal osteogenic niche for stem cell differentiation .
	manualset3
124197	1	404378	13	NULL	NULL	0	NULL	Osteopontin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Osteopontin as a marker of weight loss in lung cancer .
	manualset3
124198	2	404378	13	NULL	NULL	0	NULL	marker	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Osteopontin as a marker of weight loss in lung cancer .
	manualset3
124199	3	404378	13	NULL	NULL	0	NULL	weight loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Osteopontin as a marker of weight loss in lung cancer .
	manualset3
124200	4	404378	13	NULL	NULL	0	NULL	lung cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Osteopontin as a marker of weight loss in lung cancer .
	manualset3
124201	1	404379	13	NULL	NULL	0	NULL	antimicrobial defense 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A disturbed antimicrobial defense , as provided by Paneth and other epithelial defensins , seems to be a critical factor in the pathogenesis of inflammatory bowel diseases .
	manualset3
124202	2	404379	13	NULL	NULL	NULL	NULL	Paneth	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A disturbed antimicrobial defense , as provided by Paneth and other epithelial defensins , seems to be a critical factor in the pathogenesis of inflammatory bowel diseases .
	manualset3
124203	3	404379	13	NULL	NULL	0	NULL	epithelial defensins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A disturbed antimicrobial defense , as provided by Paneth and other epithelial defensins , seems to be a critical factor in the pathogenesis of inflammatory bowel diseases .
	manualset3
124204	4	404379	13	NULL	NULL	0	NULL	critical factor 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A disturbed antimicrobial defense , as provided by Paneth and other epithelial defensins , seems to be a critical factor in the pathogenesis of inflammatory bowel diseases .
	manualset3
124205	5	404379	13	NULL	NULL	0	NULL	pathogenesis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A disturbed antimicrobial defense , as provided by Paneth and other epithelial defensins , seems to be a critical factor in the pathogenesis of inflammatory bowel diseases .
	manualset3
124206	6	404379	13	NULL	NULL	0	NULL	inflammatory bowel diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A disturbed antimicrobial defense , as provided by Paneth and other epithelial defensins , seems to be a critical factor in the pathogenesis of inflammatory bowel diseases .
	manualset3
124207	1	404380	13	NULL	NULL	0	NULL	Ota 's nevus 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Ota 's nevus is a dermal melanocytic disease which causes serious cosmetic problems for affected individuals .
	manualset3
124208	2	404380	13	NULL	NULL	0	NULL	dermal melanocytic disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Ota 's nevus is a dermal melanocytic disease which causes serious cosmetic problems for affected individuals .
	manualset3
124209	3	404380	13	NULL	NULL	0	NULL	serious cosmetic problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ota 's nevus is a dermal melanocytic disease which causes serious cosmetic problems for affected individuals .
	manualset3
124210	4	404380	13	NULL	NULL	0	NULL	individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ota 's nevus is a dermal melanocytic disease which causes serious cosmetic problems for affected individuals .
	manualset3
124211	1	404381	13	NULL	NULL	0	NULL	adjuvant forms of therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Other adjuvant forms of therapy pre - and post-operatively must be assessed .
	manualset3
124212	1	404382	13	NULL	NULL	0	NULL	angiotensin II receptor antagonists	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Other angiotensin II receptor antagonists also inhibited PAH secretion with similar potencies : eprosartan , 11 + / - 2.3 microM ; irbesartan , 17 + / - 2.2 microM ; and valsartan 3 + / - 0.6 microM .
	manualset3
124213	2	404382	13	NULL	NULL	0	NULL	PAH secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Other angiotensin II receptor antagonists also inhibited PAH secretion with similar potencies : eprosartan , 11 + / - 2.3 microM ; irbesartan , 17 + / - 2.2 microM ; and valsartan 3 + / - 0.6 microM .
	manualset3
124214	3	404382	13	NULL	NULL	0	NULL	potencies	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Other angiotensin II receptor antagonists also inhibited PAH secretion with similar potencies : eprosartan , 11 + / - 2.3 microM ; irbesartan , 17 + / - 2.2 microM ; and valsartan 3 + / - 0.6 microM .
	manualset3
124215	4	404382	13	NULL	NULL	0	NULL	eprosartan	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Other angiotensin II receptor antagonists also inhibited PAH secretion with similar potencies : eprosartan , 11 + / - 2.3 microM ; irbesartan , 17 + / - 2.2 microM ; and valsartan 3 + / - 0.6 microM .
	manualset3
124216	5	404382	13	NULL	NULL	0	NULL	11 + / - 2.3 microM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Other angiotensin II receptor antagonists also inhibited PAH secretion with similar potencies : eprosartan , 11 + / - 2.3 microM ; irbesartan , 17 + / - 2.2 microM ; and valsartan 3 + / - 0.6 microM .
	manualset3
124217	6	404382	13	NULL	NULL	0	NULL	irbesartan	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Other angiotensin II receptor antagonists also inhibited PAH secretion with similar potencies : eprosartan , 11 + / - 2.3 microM ; irbesartan , 17 + / - 2.2 microM ; and valsartan 3 + / - 0.6 microM .
	manualset3
124218	7	404382	13	NULL	NULL	0	NULL	17 + / - 2.2 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Other angiotensin II receptor antagonists also inhibited PAH secretion with similar potencies : eprosartan , 11 + / - 2.3 microM ; irbesartan , 17 + / - 2.2 microM ; and valsartan 3 + / - 0.6 microM .
	manualset3
124219	8	404382	13	NULL	NULL	0	NULL	valsartan	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Other angiotensin II receptor antagonists also inhibited PAH secretion with similar potencies : eprosartan , 11 + / - 2.3 microM ; irbesartan , 17 + / - 2.2 microM ; and valsartan 3 + / - 0.6 microM .
	manualset3
124220	9	404382	13	NULL	NULL	0	NULL	3 + / - 0.6 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Other angiotensin II receptor antagonists also inhibited PAH secretion with similar potencies : eprosartan , 11 + / - 2.3 microM ; irbesartan , 17 + / - 2.2 microM ; and valsartan 3 + / - 0.6 microM .
	manualset3
124221	1	404383	13	NULL	NULL	0	NULL	bat species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Other bat species were tested for the presence of this repetitive DNA .
	manualset3
124222	2	404383	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Other bat species were tested for the presence of this repetitive DNA .
	manualset3
124223	3	404383	13	NULL	NULL	0	NULL	repetitive DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Other bat species were tested for the presence of this repetitive DNA .
	manualset3
124224	1	404384	13	NULL	NULL	0	NULL	enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Other enzymes that transfer a methyl group to carbon 5 of a pyrimidine nucleotide , such as the bacterial DNA m ( 5 ) C methyltransferases , utilize their single conserved cysteine residue to form a covalent Michael adduct with carbon 6 of the pyrimidine ring during catalysis .
	manualset3
124225	2	404384	13	NULL	NULL	0	NULL	transfer	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Other enzymes that transfer a methyl group to carbon 5 of a pyrimidine nucleotide , such as the bacterial DNA m ( 5 ) C methyltransferases , utilize their single conserved cysteine residue to form a covalent Michael adduct with carbon 6 of the pyrimidine ring during catalysis .
	manualset3
124226	3	404384	13	NULL	NULL	0	NULL	methyl group 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Other enzymes that transfer a methyl group to carbon 5 of a pyrimidine nucleotide , such as the bacterial DNA m ( 5 ) C methyltransferases , utilize their single conserved cysteine residue to form a covalent Michael adduct with carbon 6 of the pyrimidine ring during catalysis .
	manualset3
124227	4	404384	13	NULL	NULL	0	NULL	carbon 5	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Other enzymes that transfer a methyl group to carbon 5 of a pyrimidine nucleotide , such as the bacterial DNA m ( 5 ) C methyltransferases , utilize their single conserved cysteine residue to form a covalent Michael adduct with carbon 6 of the pyrimidine ring during catalysis .
	manualset3
124228	5	404384	13	NULL	NULL	0	NULL	pyrimidine nucleotide	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Other enzymes that transfer a methyl group to carbon 5 of a pyrimidine nucleotide , such as the bacterial DNA m ( 5 ) C methyltransferases , utilize their single conserved cysteine residue to form a covalent Michael adduct with carbon 6 of the pyrimidine ring during catalysis .
	manualset3
124229	6	404384	13	NULL	NULL	0	NULL	bacterial DNA m ( 5 ) C methyltransferases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Other enzymes that transfer a methyl group to carbon 5 of a pyrimidine nucleotide , such as the bacterial DNA m ( 5 ) C methyltransferases , utilize their single conserved cysteine residue to form a covalent Michael adduct with carbon 6 of the pyrimidine ring during catalysis .
	manualset3
124230	7	404384	13	NULL	NULL	0	NULL	cysteine residue	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Other enzymes that transfer a methyl group to carbon 5 of a pyrimidine nucleotide , such as the bacterial DNA m ( 5 ) C methyltransferases , utilize their single conserved cysteine residue to form a covalent Michael adduct with carbon 6 of the pyrimidine ring during catalysis .
	manualset3
124231	8	404384	13	NULL	NULL	0	NULL	covalent Michael adduct	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Other enzymes that transfer a methyl group to carbon 5 of a pyrimidine nucleotide , such as the bacterial DNA m ( 5 ) C methyltransferases , utilize their single conserved cysteine residue to form a covalent Michael adduct with carbon 6 of the pyrimidine ring during catalysis .
	manualset3
124232	9	404384	13	NULL	NULL	0	NULL	carbon 6	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Other enzymes that transfer a methyl group to carbon 5 of a pyrimidine nucleotide , such as the bacterial DNA m ( 5 ) C methyltransferases , utilize their single conserved cysteine residue to form a covalent Michael adduct with carbon 6 of the pyrimidine ring during catalysis .
	manualset3
124233	10	404384	13	NULL	NULL	0	NULL	pyrimidine ring	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Other enzymes that transfer a methyl group to carbon 5 of a pyrimidine nucleotide , such as the bacterial DNA m ( 5 ) C methyltransferases , utilize their single conserved cysteine residue to form a covalent Michael adduct with carbon 6 of the pyrimidine ring during catalysis .
	manualset3
124235	11	404384	13	NULL	NULL	0	NULL	catalysis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Other enzymes that transfer a methyl group to carbon 5 of a pyrimidine nucleotide , such as the bacterial DNA m ( 5 ) C methyltransferases , utilize their single conserved cysteine residue to form a covalent Michael adduct with carbon 6 of the pyrimidine ring during catalysis .
	manualset3
124237	1	404385	13	NULL	NULL	0	NULL	factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Other factors are also considered such that end users may better select the optimum spectrograph for their particular application .
	manualset3
124238	2	404385	13	NULL	NULL	0	NULL	end users	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Other factors are also considered such that end users may better select the optimum spectrograph for their particular application .
	manualset3
124241	3	404385	13	NULL	NULL	0	NULL	optimum spectrograph 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Other factors are also considered such that end users may better select the optimum spectrograph for their particular application .
	manualset3
124242	4	404385	13	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Other factors are also considered such that end users may better select the optimum spectrograph for their particular application .
	manualset3
124243	1	404386	13	NULL	NULL	NULL	NULL	factors	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Other factors influencing sodium or chloride transport are likely to be the cause of the symptoms in the patient described .
	manualset3
124245	2	404386	13	NULL	NULL	0	NULL	sodium transport 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Other factors influencing sodium or chloride transport are likely to be the cause of the symptoms in the patient described .
	manualset3
124246	3	404386	13	NULL	NULL	0	NULL	chloride transport 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Other factors influencing sodium or chloride transport are likely to be the cause of the symptoms in the patient described .
	manualset3
124247	4	404386	13	NULL	NULL	0	NULL	cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Other factors influencing sodium or chloride transport are likely to be the cause of the symptoms in the patient described .
	manualset3
124248	5	404386	13	NULL	NULL	0	NULL	symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Other factors influencing sodium or chloride transport are likely to be the cause of the symptoms in the patient described .
	manualset3
124249	6	404386	13	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Other factors influencing sodium or chloride transport are likely to be the cause of the symptoms in the patient described .
	manualset3
124250	1	404387	13	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Other genes that were significantly upregulated included Fmo2 and peroxiredoxins , whereas genes downregulated included Catalase and Serpinb1b .
	manualset3
124251	2	404387	13	NULL	NULL	0	NULL	Fmo2 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Other genes that were significantly upregulated included Fmo2 and peroxiredoxins , whereas genes downregulated included Catalase and Serpinb1b .
	manualset3
124252	3	404387	13	NULL	NULL	0	NULL	peroxiredoxins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Other genes that were significantly upregulated included Fmo2 and peroxiredoxins , whereas genes downregulated included Catalase and Serpinb1b .
	manualset3
124253	4	404387	13	NULL	NULL	0	NULL	genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Other genes that were significantly upregulated included Fmo2 and peroxiredoxins , whereas genes downregulated included Catalase and Serpinb1b .
	manualset3
124254	5	404387	13	NULL	NULL	0	NULL	Catalase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Other genes that were significantly upregulated included Fmo2 and peroxiredoxins , whereas genes downregulated included Catalase and Serpinb1b .
	manualset3
124255	6	404387	13	NULL	NULL	0	NULL	Serpinb1b 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Other genes that were significantly upregulated included Fmo2 and peroxiredoxins , whereas genes downregulated included Catalase and Serpinb1b .
	manualset3
124256	1	404388	13	NULL	NULL	0	NULL	immunodeficiencies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Other immunodeficiencies that may soon be amenable to somatic gene therapy include leukocyte adhesion deficiency and chronic granulomatous disease .
	manualset3
124257	2	404388	13	NULL	NULL	0	NULL	somatic gene therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Other immunodeficiencies that may soon be amenable to somatic gene therapy include leukocyte adhesion deficiency and chronic granulomatous disease .
	manualset3
124258	3	404388	13	NULL	NULL	0	NULL	leukocyte adhesion deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Other immunodeficiencies that may soon be amenable to somatic gene therapy include leukocyte adhesion deficiency and chronic granulomatous disease .
	manualset3
124259	4	404388	13	NULL	NULL	0	NULL	chronic granulomatous disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Other immunodeficiencies that may soon be amenable to somatic gene therapy include leukocyte adhesion deficiency and chronic granulomatous disease .
	manualset3
124260	1	404389	13	NULL	NULL	0	NULL	leaching tests 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Other leaching tests such as NEN 7341 test , ANS 16.1 and multiple TCLP ( MTCLP ) test conducted on select solidified blocks showed that chromium was immobilized by the binder studied .
	manualset3
124261	2	404389	13	NULL	NULL	0	NULL	NEN 7341 test 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Other leaching tests such as NEN 7341 test , ANS 16.1 and multiple TCLP ( MTCLP ) test conducted on select solidified blocks showed that chromium was immobilized by the binder studied .
	manualset3
124262	3	404389	13	NULL	NULL	0	NULL	ANS 16.1 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Other leaching tests such as NEN 7341 test , ANS 16.1 and multiple TCLP ( MTCLP ) test conducted on select solidified blocks showed that chromium was immobilized by the binder studied .
	manualset3
124263	4	404389	13	NULL	NULL	0	NULL	multiple TCLP ( MTCLP ) test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Other leaching tests such as NEN 7341 test , ANS 16.1 and multiple TCLP ( MTCLP ) test conducted on select solidified blocks showed that chromium was immobilized by the binder studied .
	manualset3
124264	5	404389	13	NULL	NULL	0	NULL	blocks 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Other leaching tests such as NEN 7341 test , ANS 16.1 and multiple TCLP ( MTCLP ) test conducted on select solidified blocks showed that chromium was immobilized by the binder studied .
	manualset3
124265	6	404389	13	NULL	NULL	0	NULL	chromium 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Other leaching tests such as NEN 7341 test , ANS 16.1 and multiple TCLP ( MTCLP ) test conducted on select solidified blocks showed that chromium was immobilized by the binder studied .
	manualset3
124266	7	404389	13	NULL	NULL	0	NULL	binder	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Other leaching tests such as NEN 7341 test , ANS 16.1 and multiple TCLP ( MTCLP ) test conducted on select solidified blocks showed that chromium was immobilized by the binder studied .
	manualset3
124267	1	404390	13	NULL	NULL	0	NULL	members	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Other members of the T-type calcium channel family were also regulated by syntaxin-1A , but to a smaller extent .
	manualset3
124268	2	404390	13	NULL	NULL	0	NULL	T-type calcium channel family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Other members of the T-type calcium channel family were also regulated by syntaxin-1A , but to a smaller extent .
	manualset3
124269	3	404390	13	NULL	NULL	0	NULL	syntaxin-1A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Other members of the T-type calcium channel family were also regulated by syntaxin-1A , but to a smaller extent .
	manualset3
124270	4	404390	13	NULL	NULL	0	NULL	extent	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Other members of the T-type calcium channel family were also regulated by syntaxin-1A , but to a smaller extent .
	manualset3
124271	1	404391	13	NULL	NULL	0	NULL	nerve terminal components	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Other nerve terminal components are absent from this complex .
	manualset3
124272	2	404391	13	NULL	NULL	0	NULL	complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Other nerve terminal components are absent from this complex .
	manualset3
124273	1	404392	13	NULL	NULL	0	NULL	 neurotransmitter systems	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Other neurotransmitter systems having minor influence on cognitive functions - as shown by the weakness of the effects of their selective lesions - modulate cholinergic functions .
	manualset3
124274	2	404392	13	NULL	NULL	0	NULL	influence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Other neurotransmitter systems having minor influence on cognitive functions - as shown by the weakness of the effects of their selective lesions - modulate cholinergic functions .
	manualset3
124275	3	404392	13	NULL	NULL	0	NULL	cognitive functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Other neurotransmitter systems having minor influence on cognitive functions - as shown by the weakness of the effects of their selective lesions - modulate cholinergic functions .
	manualset3
124276	4	404392	13	NULL	NULL	0	NULL	weakness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Other neurotransmitter systems having minor influence on cognitive functions - as shown by the weakness of the effects of their selective lesions - modulate cholinergic functions .
	manualset3
124277	5	404392	13	NULL	NULL	0	NULL	effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Other neurotransmitter systems having minor influence on cognitive functions - as shown by the weakness of the effects of their selective lesions - modulate cholinergic functions .
	manualset3
124278	6	404392	13	NULL	NULL	0	NULL	lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Other neurotransmitter systems having minor influence on cognitive functions - as shown by the weakness of the effects of their selective lesions - modulate cholinergic functions .
	manualset3
124279	7	404392	13	NULL	NULL	NULL	NULL	cholinergic functions	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Other neurotransmitter systems having minor influence on cognitive functions - as shown by the weakness of the effects of their selective lesions - modulate cholinergic functions .
	manualset3
124280	1	404393	13	NULL	NULL	0	NULL	participants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Other participants pointed out that major cultural and economic changes need to take place before males will assume more responsibility for their role in reproduction .
	manualset3
124281	2	404393	13	NULL	NULL	0	NULL	major cultural changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Other participants pointed out that major cultural and economic changes need to take place before males will assume more responsibility for their role in reproduction .
	manualset3
124282	3	404393	13	NULL	NULL	0	NULL	economic changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Other participants pointed out that major cultural and economic changes need to take place before males will assume more responsibility for their role in reproduction .
	manualset3
124283	4	404393	13	NULL	NULL	0	NULL	males	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Other participants pointed out that major cultural and economic changes need to take place before males will assume more responsibility for their role in reproduction .
	manualset3
124284	5	404393	13	NULL	NULL	0	NULL	responsibility	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Other participants pointed out that major cultural and economic changes need to take place before males will assume more responsibility for their role in reproduction .
	manualset3
124285	6	404393	13	NULL	NULL	0	NULL	role 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Other participants pointed out that major cultural and economic changes need to take place before males will assume more responsibility for their role in reproduction .
	manualset3
124286	7	404393	13	NULL	NULL	0	NULL	reproduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Other participants pointed out that major cultural and economic changes need to take place before males will assume more responsibility for their role in reproduction .
	manualset3
124287	1	404394	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Other patients with CRPS may have related neurocognitive defects .
	manualset3
124288	2	404394	13	NULL	NULL	0	NULL	CRPS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Other patients with CRPS may have related neurocognitive defects .
	manualset3
124289	3	404394	13	NULL	NULL	0	NULL	neurocognitive defects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Other patients with CRPS may have related neurocognitive defects .
	manualset3
124290	1	404395	13	NULL	NULL	0	NULL	people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Other people , chance happenings , physical discomfort , and perceptions of fitness , weight , and appearance played a role in whether the subjects exercised .
	manualset3
124291	2	404395	13	NULL	NULL	0	NULL	chance happenings 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Other people , chance happenings , physical discomfort , and perceptions of fitness , weight , and appearance played a role in whether the subjects exercised .
	manualset3
124292	3	404395	13	NULL	NULL	0	NULL	physical discomfort 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Other people , chance happenings , physical discomfort , and perceptions of fitness , weight , and appearance played a role in whether the subjects exercised .
	manualset3
124293	4	404395	13	NULL	NULL	0	NULL	perceptions of fitness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Other people , chance happenings , physical discomfort , and perceptions of fitness , weight , and appearance played a role in whether the subjects exercised .
	manualset3
124294	5	404395	13	NULL	NULL	0	NULL	weight	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Other people , chance happenings , physical discomfort , and perceptions of fitness , weight , and appearance played a role in whether the subjects exercised .
	manualset3
124295	6	404395	13	NULL	NULL	0	NULL	appearance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Other people , chance happenings , physical discomfort , and perceptions of fitness , weight , and appearance played a role in whether the subjects exercised .
	manualset3
124296	7	404395	13	NULL	NULL	0	NULL	role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Other people , chance happenings , physical discomfort , and perceptions of fitness , weight , and appearance played a role in whether the subjects exercised .
	manualset3
124297	8	404395	13	NULL	NULL	0	NULL	subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Other people , chance happenings , physical discomfort , and perceptions of fitness , weight , and appearance played a role in whether the subjects exercised .
	manualset3
124298	1	404396	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose-related increase in the diuresis and in sodium and potassium excretion was present in both young and old rats .
	manualset3
124299	2	404396	13	NULL	NULL	0	NULL	diuresis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose-related increase in the diuresis and in sodium and potassium excretion was present in both young and old rats .
	manualset3
124300	3	404396	13	NULL	NULL	0	NULL	sodium excretion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose-related increase in the diuresis and in sodium and potassium excretion was present in both young and old rats .
	manualset3
124301	4	404396	13	NULL	NULL	0	NULL	potassium excretion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose-related increase in the diuresis and in sodium and potassium excretion was present in both young and old rats .
	manualset3
124302	5	404396	13	NULL	NULL	0	NULL	young rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose-related increase in the diuresis and in sodium and potassium excretion was present in both young and old rats .
	manualset3
124303	6	404396	13	NULL	NULL	0	NULL	old rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose-related increase in the diuresis and in sodium and potassium excretion was present in both young and old rats .
	manualset3
124304	1	404397	13	NULL	NULL	0	NULL	symptom patterns 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Other symptom patterns in patients with eating disorders , including mood dysregulation , impulsivity , and obsessionality , as well as therapeutic response to serotonergic agents , suggest involvement of serotonergic pathways .
	manualset3
124305	2	404397	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Other symptom patterns in patients with eating disorders , including mood dysregulation , impulsivity , and obsessionality , as well as therapeutic response to serotonergic agents , suggest involvement of serotonergic pathways .
	manualset3
124306	3	404397	13	NULL	NULL	0	NULL	eating disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Other symptom patterns in patients with eating disorders , including mood dysregulation , impulsivity , and obsessionality , as well as therapeutic response to serotonergic agents , suggest involvement of serotonergic pathways .
	manualset3
124307	4	404397	13	NULL	NULL	0	NULL	mood dysregulation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Other symptom patterns in patients with eating disorders , including mood dysregulation , impulsivity , and obsessionality , as well as therapeutic response to serotonergic agents , suggest involvement of serotonergic pathways .
	manualset3
124308	5	404397	13	NULL	NULL	0	NULL	impulsivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Other symptom patterns in patients with eating disorders , including mood dysregulation , impulsivity , and obsessionality , as well as therapeutic response to serotonergic agents , suggest involvement of serotonergic pathways .
	manualset3
124309	6	404397	13	NULL	NULL	0	NULL	obsessionality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Other symptom patterns in patients with eating disorders , including mood dysregulation , impulsivity , and obsessionality , as well as therapeutic response to serotonergic agents , suggest involvement of serotonergic pathways .
	manualset3
124310	7	404397	13	NULL	NULL	0	NULL	therapeutic response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Other symptom patterns in patients with eating disorders , including mood dysregulation , impulsivity , and obsessionality , as well as therapeutic response to serotonergic agents , suggest involvement of serotonergic pathways .
	manualset3
124311	8	404397	13	NULL	NULL	0	NULL	serotonergic agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Other symptom patterns in patients with eating disorders , including mood dysregulation , impulsivity , and obsessionality , as well as therapeutic response to serotonergic agents , suggest involvement of serotonergic pathways .
	manualset3
124312	9	404397	13	NULL	NULL	0	NULL	involvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Other symptom patterns in patients with eating disorders , including mood dysregulation , impulsivity , and obsessionality , as well as therapeutic response to serotonergic agents , suggest involvement of serotonergic pathways .
	manualset3
124313	10	404397	13	NULL	NULL	0	NULL	serotonergic pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Other symptom patterns in patients with eating disorders , including mood dysregulation , impulsivity , and obsessionality , as well as therapeutic response to serotonergic agents , suggest involvement of serotonergic pathways .
	manualset3
124314	1	404398	13	NULL	NULL	0	NULL	supervision 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Other than supervision of infants for jaundice , conditions requiring medical intervention were not linked to time of discharge .
	manualset3
124315	2	404398	13	NULL	NULL	0	NULL	infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Other than supervision of infants for jaundice , conditions requiring medical intervention were not linked to time of discharge .
	manualset3
124316	3	404398	13	NULL	NULL	0	NULL	jaundice 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Other than supervision of infants for jaundice , conditions requiring medical intervention were not linked to time of discharge .
	manualset3
124317	4	404398	13	NULL	NULL	0	NULL	conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Other than supervision of infants for jaundice , conditions requiring medical intervention were not linked to time of discharge .
	manualset3
124318	5	404398	13	NULL	NULL	0	NULL	intervention 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Other than supervision of infants for jaundice , conditions requiring medical intervention were not linked to time of discharge .
	manualset3
124319	6	404398	13	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Other than supervision of infants for jaundice , conditions requiring medical intervention were not linked to time of discharge .
	manualset3
124320	7	404398	13	NULL	NULL	0	NULL	discharge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Other than supervision of infants for jaundice , conditions requiring medical intervention were not linked to time of discharge .
	manualset3
124321	1	404399	13	NULL	NULL	0	NULL	variants of renal damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Other variants of renal damage in sarcoidosis , excluding amyloidosis , form the basis for corticosteroid administration even in cases of the presence of renal failure , demonstrating that so-called `` dramatic therapy '' produces a remarkable beneficial effect characterized by the disappearance of the signs of renal failure .
	manualset3
124322	2	404399	13	NULL	NULL	0	NULL	sarcoidosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Other variants of renal damage in sarcoidosis , excluding amyloidosis , form the basis for corticosteroid administration even in cases of the presence of renal failure , demonstrating that so-called `` dramatic therapy '' produces a remarkable beneficial effect characterized by the disappearance of the signs of renal failure .
	manualset3
124323	3	404399	13	NULL	NULL	0	NULL	amyloidosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Other variants of renal damage in sarcoidosis , excluding amyloidosis , form the basis for corticosteroid administration even in cases of the presence of renal failure , demonstrating that so-called `` dramatic therapy '' produces a remarkable beneficial effect characterized by the disappearance of the signs of renal failure .
	manualset3
124324	4	404399	13	NULL	NULL	0	NULL	basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Other variants of renal damage in sarcoidosis , excluding amyloidosis , form the basis for corticosteroid administration even in cases of the presence of renal failure , demonstrating that so-called `` dramatic therapy '' produces a remarkable beneficial effect characterized by the disappearance of the signs of renal failure .
	manualset3
124325	5	404399	13	NULL	NULL	0	NULL	corticosteroid administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Other variants of renal damage in sarcoidosis , excluding amyloidosis , form the basis for corticosteroid administration even in cases of the presence of renal failure , demonstrating that so-called `` dramatic therapy '' produces a remarkable beneficial effect characterized by the disappearance of the signs of renal failure .
	manualset3
124326	6	404399	13	NULL	NULL	0	NULL	cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Other variants of renal damage in sarcoidosis , excluding amyloidosis , form the basis for corticosteroid administration even in cases of the presence of renal failure , demonstrating that so-called `` dramatic therapy '' produces a remarkable beneficial effect characterized by the disappearance of the signs of renal failure .
	manualset3
124327	7	404399	13	NULL	NULL	0	NULL	presence of renal failure 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Other variants of renal damage in sarcoidosis , excluding amyloidosis , form the basis for corticosteroid administration even in cases of the presence of renal failure , demonstrating that so-called `` dramatic therapy '' produces a remarkable beneficial effect characterized by the disappearance of the signs of renal failure .
	manualset3
124328	8	404399	13	NULL	NULL	0	NULL	dramatic therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Other variants of renal damage in sarcoidosis , excluding amyloidosis , form the basis for corticosteroid administration even in cases of the presence of renal failure , demonstrating that so-called `` dramatic therapy '' produces a remarkable beneficial effect characterized by the disappearance of the signs of renal failure .
	manualset3
124329	9	404399	13	NULL	NULL	0	NULL	beneficial effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Other variants of renal damage in sarcoidosis , excluding amyloidosis , form the basis for corticosteroid administration even in cases of the presence of renal failure , demonstrating that so-called `` dramatic therapy '' produces a remarkable beneficial effect characterized by the disappearance of the signs of renal failure .
	manualset3
124330	10	404399	13	NULL	NULL	0	NULL	disappearance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Other variants of renal damage in sarcoidosis , excluding amyloidosis , form the basis for corticosteroid administration even in cases of the presence of renal failure , demonstrating that so-called `` dramatic therapy '' produces a remarkable beneficial effect characterized by the disappearance of the signs of renal failure .
	manualset3
124331	11	404399	13	NULL	NULL	0	NULL	signs of renal failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Other variants of renal damage in sarcoidosis , excluding amyloidosis , form the basis for corticosteroid administration even in cases of the presence of renal failure , demonstrating that so-called `` dramatic therapy '' produces a remarkable beneficial effect characterized by the disappearance of the signs of renal failure .
	manualset3
124332	1	404400	13	NULL	NULL	0	NULL	Others	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Others have failed to show any superiority to placebo treatment when tested in controlled drug trials for a period long enough to rule out the placebo response , which may simulate effectiveness at the beginning of the trial .
	manualset3
124333	2	404400	13	NULL	NULL	0	NULL	placebo treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Others have failed to show any superiority to placebo treatment when tested in controlled drug trials for a period long enough to rule out the placebo response , which may simulate effectiveness at the beginning of the trial .
	manualset3
124334	3	404400	13	NULL	NULL	0	NULL	drug trials 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Others have failed to show any superiority to placebo treatment when tested in controlled drug trials for a period long enough to rule out the placebo response , which may simulate effectiveness at the beginning of the trial .
	manualset3
124335	4	404400	13	NULL	NULL	0	NULL	period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Others have failed to show any superiority to placebo treatment when tested in controlled drug trials for a period long enough to rule out the placebo response , which may simulate effectiveness at the beginning of the trial .
	manualset3
124336	5	404400	13	NULL	NULL	0	NULL	placebo response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Others have failed to show any superiority to placebo treatment when tested in controlled drug trials for a period long enough to rule out the placebo response , which may simulate effectiveness at the beginning of the trial .
	manualset3
124337	6	404400	13	NULL	NULL	0	NULL	effectiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Others have failed to show any superiority to placebo treatment when tested in controlled drug trials for a period long enough to rule out the placebo response , which may simulate effectiveness at the beginning of the trial .
	manualset3
124338	7	404400	13	NULL	NULL	0	NULL	trial	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Others have failed to show any superiority to placebo treatment when tested in controlled drug trials for a period long enough to rule out the placebo response , which may simulate effectiveness at the beginning of the trial .
	manualset3
124339	8	404400	13	NULL	NULL	0	NULL	beginning 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Others have failed to show any superiority to placebo treatment when tested in controlled drug trials for a period long enough to rule out the placebo response , which may simulate effectiveness at the beginning of the trial .
	manualset3
124454	1	404401	13	NULL	NULL	0	NULL	salt	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Otherwise , salt , chilling , abscisic acid and jasmonic acid triggered a significant induction ( more than tenfold ) of PgSPD within 12-24 h post-treatment , especially ; PgSPD was prominently induced by salt ( 41.5-fold ) .
	manualset3
124455	2	404401	13	NULL	NULL	0	NULL	abscisic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Otherwise , salt , chilling , abscisic acid and jasmonic acid triggered a significant induction ( more than tenfold ) of PgSPD within 12-24 h post-treatment , especially ; PgSPD was prominently induced by salt ( 41.5-fold ) .
	manualset3
124456	3	404401	13	NULL	NULL	0	NULL	jasmonic acid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Otherwise , salt , chilling , abscisic acid and jasmonic acid triggered a significant induction ( more than tenfold ) of PgSPD within 12-24 h post-treatment , especially ; PgSPD was prominently induced by salt ( 41.5-fold ) .
	manualset3
124457	4	404401	13	NULL	NULL	0	NULL	induction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Otherwise , salt , chilling , abscisic acid and jasmonic acid triggered a significant induction ( more than tenfold ) of PgSPD within 12-24 h post-treatment , especially ; PgSPD was prominently induced by salt ( 41.5-fold ) .
	manualset3
124458	5	404401	13	NULL	NULL	0	NULL	PgSPD	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Otherwise , salt , chilling , abscisic acid and jasmonic acid triggered a significant induction ( more than tenfold ) of PgSPD within 12-24 h post-treatment , especially ; PgSPD was prominently induced by salt ( 41.5-fold ) .
	manualset3
124459	6	404401	13	NULL	NULL	0	NULL	12-24 h 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Otherwise , salt , chilling , abscisic acid and jasmonic acid triggered a significant induction ( more than tenfold ) of PgSPD within 12-24 h post-treatment , especially ; PgSPD was prominently induced by salt ( 41.5-fold ) .
	manualset3
124460	7	404401	13	NULL	NULL	0	NULL	PgSPD	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Otherwise , salt , chilling , abscisic acid and jasmonic acid triggered a significant induction ( more than tenfold ) of PgSPD within 12-24 h post-treatment , especially ; PgSPD was prominently induced by salt ( 41.5-fold ) .
	manualset3
124461	8	404401	13	NULL	NULL	0	NULL	salt	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Otherwise , salt , chilling , abscisic acid and jasmonic acid triggered a significant induction ( more than tenfold ) of PgSPD within 12-24 h post-treatment , especially ; PgSPD was prominently induced by salt ( 41.5-fold ) .
	manualset3
124462	9	404401	13	NULL	NULL	0	NULL	41.5-fold	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Otherwise , salt , chilling , abscisic acid and jasmonic acid triggered a significant induction ( more than tenfold ) of PgSPD within 12-24 h post-treatment , especially ; PgSPD was prominently induced by salt ( 41.5-fold ) .
	manualset3
124463	1	404402	13	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our aim was to evaluate the role of changes in circulating levels of soluble Fas ( sFas ) , suggestive of an enhanced inhibitory response to ongoing apoptosis , and soluble IL2 receptor ( sIL2-R ) , indicative of T-lymphocyte activation , in chronic heart failure and unstable angina pectoris .
	manualset3
124464	2	404402	13	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our aim was to evaluate the role of changes in circulating levels of soluble Fas ( sFas ) , suggestive of an enhanced inhibitory response to ongoing apoptosis , and soluble IL2 receptor ( sIL2-R ) , indicative of T-lymphocyte activation , in chronic heart failure and unstable angina pectoris .
	manualset3
124465	3	404402	13	NULL	NULL	0	NULL	changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our aim was to evaluate the role of changes in circulating levels of soluble Fas ( sFas ) , suggestive of an enhanced inhibitory response to ongoing apoptosis , and soluble IL2 receptor ( sIL2-R ) , indicative of T-lymphocyte activation , in chronic heart failure and unstable angina pectoris .
	manualset3
124466	4	404402	13	NULL	NULL	0	NULL	levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our aim was to evaluate the role of changes in circulating levels of soluble Fas ( sFas ) , suggestive of an enhanced inhibitory response to ongoing apoptosis , and soluble IL2 receptor ( sIL2-R ) , indicative of T-lymphocyte activation , in chronic heart failure and unstable angina pectoris .
	manualset3
124467	5	404402	13	NULL	NULL	0	NULL	soluble Fas ( sFas ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our aim was to evaluate the role of changes in circulating levels of soluble Fas ( sFas ) , suggestive of an enhanced inhibitory response to ongoing apoptosis , and soluble IL2 receptor ( sIL2-R ) , indicative of T-lymphocyte activation , in chronic heart failure and unstable angina pectoris .
	manualset3
124468	6	404402	13	NULL	NULL	0	NULL	inhibitory response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our aim was to evaluate the role of changes in circulating levels of soluble Fas ( sFas ) , suggestive of an enhanced inhibitory response to ongoing apoptosis , and soluble IL2 receptor ( sIL2-R ) , indicative of T-lymphocyte activation , in chronic heart failure and unstable angina pectoris .
	manualset3
124469	7	404402	13	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our aim was to evaluate the role of changes in circulating levels of soluble Fas ( sFas ) , suggestive of an enhanced inhibitory response to ongoing apoptosis , and soluble IL2 receptor ( sIL2-R ) , indicative of T-lymphocyte activation , in chronic heart failure and unstable angina pectoris .
	manualset3
124470	8	404402	13	NULL	NULL	0	NULL	soluble IL2 receptor ( sIL2-R )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our aim was to evaluate the role of changes in circulating levels of soluble Fas ( sFas ) , suggestive of an enhanced inhibitory response to ongoing apoptosis , and soluble IL2 receptor ( sIL2-R ) , indicative of T-lymphocyte activation , in chronic heart failure and unstable angina pectoris .
	manualset3
124471	9	404402	13	NULL	NULL	0	NULL	T-lymphocyte activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our aim was to evaluate the role of changes in circulating levels of soluble Fas ( sFas ) , suggestive of an enhanced inhibitory response to ongoing apoptosis , and soluble IL2 receptor ( sIL2-R ) , indicative of T-lymphocyte activation , in chronic heart failure and unstable angina pectoris .
	manualset3
124472	10	404402	13	NULL	NULL	0	NULL	chronic heart failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our aim was to evaluate the role of changes in circulating levels of soluble Fas ( sFas ) , suggestive of an enhanced inhibitory response to ongoing apoptosis , and soluble IL2 receptor ( sIL2-R ) , indicative of T-lymphocyte activation , in chronic heart failure and unstable angina pectoris .
	manualset3
124473	11	404402	13	NULL	NULL	0	NULL	angina pectoris	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our aim was to evaluate the role of changes in circulating levels of soluble Fas ( sFas ) , suggestive of an enhanced inhibitory response to ongoing apoptosis , and soluble IL2 receptor ( sIL2-R ) , indicative of T-lymphocyte activation , in chronic heart failure and unstable angina pectoris .
	manualset3
124474	1	404403	13	NULL	NULL	0	NULL	analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our analyses indicate that the gp70 membrane envelope glycoproteins of certain ecotropic MuLVs contain seven oligosaccharides , whereas the GIX + antigen-containing variant gp70 contains one fewer Asn-X-Thr-linked oligosaccharide .
	manualset3
124475	2	404403	13	NULL	NULL	0	NULL	gp70 membrane envelope glycoproteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our analyses indicate that the gp70 membrane envelope glycoproteins of certain ecotropic MuLVs contain seven oligosaccharides , whereas the GIX + antigen-containing variant gp70 contains one fewer Asn-X-Thr-linked oligosaccharide .
	manualset3
124476	3	404403	13	NULL	NULL	0	NULL	ecotropic MuLVs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our analyses indicate that the gp70 membrane envelope glycoproteins of certain ecotropic MuLVs contain seven oligosaccharides , whereas the GIX + antigen-containing variant gp70 contains one fewer Asn-X-Thr-linked oligosaccharide .
	manualset3
124477	4	404403	13	NULL	NULL	0	NULL	seven	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our analyses indicate that the gp70 membrane envelope glycoproteins of certain ecotropic MuLVs contain seven oligosaccharides , whereas the GIX + antigen-containing variant gp70 contains one fewer Asn-X-Thr-linked oligosaccharide .
	manualset3
124478	5	404403	13	NULL	NULL	0	NULL	oligosaccharides 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our analyses indicate that the gp70 membrane envelope glycoproteins of certain ecotropic MuLVs contain seven oligosaccharides , whereas the GIX + antigen-containing variant gp70 contains one fewer Asn-X-Thr-linked oligosaccharide .
	manualset3
124479	6	404403	13	NULL	NULL	0	NULL	GIX + antigen-containing variant gp70	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our analyses indicate that the gp70 membrane envelope glycoproteins of certain ecotropic MuLVs contain seven oligosaccharides , whereas the GIX + antigen-containing variant gp70 contains one fewer Asn-X-Thr-linked oligosaccharide .
	manualset3
124480	7	404403	13	NULL	NULL	0	NULL	Asn-X-Thr-linked oligosaccharide	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our analyses indicate that the gp70 membrane envelope glycoproteins of certain ecotropic MuLVs contain seven oligosaccharides , whereas the GIX + antigen-containing variant gp70 contains one fewer Asn-X-Thr-linked oligosaccharide .
	manualset3
124481	1	404404	13	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our analysis indicated that the observed wide range of autosomal divergence is simply due to the coalescent process in the large ancestral population of the two species .
	manualset3
124482	2	404404	13	NULL	NULL	0	NULL	wide range	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our analysis indicated that the observed wide range of autosomal divergence is simply due to the coalescent process in the large ancestral population of the two species .
	manualset3
124483	3	404404	13	NULL	NULL	0	NULL	autosomal divergence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our analysis indicated that the observed wide range of autosomal divergence is simply due to the coalescent process in the large ancestral population of the two species .
	manualset3
124484	4	404404	13	NULL	NULL	0	NULL	coalescent process	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our analysis indicated that the observed wide range of autosomal divergence is simply due to the coalescent process in the large ancestral population of the two species .
	manualset3
124485	5	404404	13	NULL	NULL	0	NULL	large ancestral population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our analysis indicated that the observed wide range of autosomal divergence is simply due to the coalescent process in the large ancestral population of the two species .
	manualset3
124486	6	404404	13	NULL	NULL	0	NULL	two species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our analysis indicated that the observed wide range of autosomal divergence is simply due to the coalescent process in the large ancestral population of the two species .
	manualset3
124487	1	404405	13	NULL	NULL	0	NULL	calculations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our calculations suggest that this amount of tubulin would form a microtubule 1.9 cm in length if totally assembled .
	manualset3
124488	2	404405	13	NULL	NULL	0	NULL	amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our calculations suggest that this amount of tubulin would form a microtubule 1.9 cm in length if totally assembled .
	manualset3
124489	3	404405	13	NULL	NULL	0	NULL	tubulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our calculations suggest that this amount of tubulin would form a microtubule 1.9 cm in length if totally assembled .
	manualset3
124490	4	404405	13	NULL	NULL	0	NULL	microtubule 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Our calculations suggest that this amount of tubulin would form a microtubule 1.9 cm in length if totally assembled .
	manualset3
124491	5	404405	13	NULL	NULL	0	NULL	1.9 cm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our calculations suggest that this amount of tubulin would form a microtubule 1.9 cm in length if totally assembled .
	manualset3
124492	6	404405	13	NULL	NULL	0	NULL	length 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our calculations suggest that this amount of tubulin would form a microtubule 1.9 cm in length if totally assembled .
	manualset3
124493	1	404406	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data are consistent with the hypothesis that membrane fusion proceeds through highly bent membrane intermediates ( stalks ) having a net negative curvature .
	manualset3
124494	2	404406	13	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data are consistent with the hypothesis that membrane fusion proceeds through highly bent membrane intermediates ( stalks ) having a net negative curvature .
	manualset3
124495	3	404406	13	NULL	NULL	0	NULL	membrane fusion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data are consistent with the hypothesis that membrane fusion proceeds through highly bent membrane intermediates ( stalks ) having a net negative curvature .
	manualset3
124497	5	404406	13	NULL	NULL	0	NULL	membrane intermediates ( stalks ) 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data are consistent with the hypothesis that membrane fusion proceeds through highly bent membrane intermediates ( stalks ) having a net negative curvature .
	manualset3
124498	6	404406	13	NULL	NULL	0	NULL	curvature	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data are consistent with the hypothesis that membrane fusion proceeds through highly bent membrane intermediates ( stalks ) having a net negative curvature .
	manualset3
124499	1	404407	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data define a PKCiota-Par6alpha-Rac1 signaling axis that drives anchorage-independent growth and invasion of NSCLC cells through induction of MMP-10 expression .
	manualset3
124500	2	404407	13	NULL	NULL	0	NULL	PKCiota-Par6alpha-Rac1 signaling axis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data define a PKCiota-Par6alpha-Rac1 signaling axis that drives anchorage-independent growth and invasion of NSCLC cells through induction of MMP-10 expression .
	manualset3
124501	3	404407	13	NULL	NULL	0	NULL	anchorage-independent growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data define a PKCiota-Par6alpha-Rac1 signaling axis that drives anchorage-independent growth and invasion of NSCLC cells through induction of MMP-10 expression .
	manualset3
124502	4	404407	13	NULL	NULL	0	NULL	invasion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data define a PKCiota-Par6alpha-Rac1 signaling axis that drives anchorage-independent growth and invasion of NSCLC cells through induction of MMP-10 expression .
	manualset3
124503	5	404407	13	NULL	NULL	0	NULL	NSCLC cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data define a PKCiota-Par6alpha-Rac1 signaling axis that drives anchorage-independent growth and invasion of NSCLC cells through induction of MMP-10 expression .
	manualset3
124504	6	404407	13	NULL	NULL	0	NULL	induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data define a PKCiota-Par6alpha-Rac1 signaling axis that drives anchorage-independent growth and invasion of NSCLC cells through induction of MMP-10 expression .
	manualset3
124505	7	404407	13	NULL	NULL	0	NULL	MMP-10 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data define a PKCiota-Par6alpha-Rac1 signaling axis that drives anchorage-independent growth and invasion of NSCLC cells through induction of MMP-10 expression .
	manualset3
124506	1	404408	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data demonstrate that SL76002 , by altering the GABA levels , probably influences DA functioning in the corpus striatum , a region responsible for involuntary movements .
	manualset3
124507	2	404408	13	NULL	NULL	0	NULL	SL76002	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data demonstrate that SL76002 , by altering the GABA levels , probably influences DA functioning in the corpus striatum , a region responsible for involuntary movements .
	manualset3
124508	3	404408	13	NULL	NULL	0	NULL	GABA levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data demonstrate that SL76002 , by altering the GABA levels , probably influences DA functioning in the corpus striatum , a region responsible for involuntary movements .
	manualset3
124509	4	404408	13	NULL	NULL	NULL	NULL	DA functioning	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our data demonstrate that SL76002 , by altering the GABA levels , probably influences DA functioning in the corpus striatum , a region responsible for involuntary movements .
	manualset3
124510	5	404408	13	NULL	NULL	0	NULL	corpus striatum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data demonstrate that SL76002 , by altering the GABA levels , probably influences DA functioning in the corpus striatum , a region responsible for involuntary movements .
	manualset3
124511	6	404408	13	NULL	NULL	0	NULL	region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data demonstrate that SL76002 , by altering the GABA levels , probably influences DA functioning in the corpus striatum , a region responsible for involuntary movements .
	manualset3
124512	7	404408	13	NULL	NULL	0	NULL	involuntary movements 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data demonstrate that SL76002 , by altering the GABA levels , probably influences DA functioning in the corpus striatum , a region responsible for involuntary movements .
	manualset3
124513	1	404409	13	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that CIS and superficial , noninvasive papillary TCCs strongly express E-CD .
	manualset3
124514	2	404409	13	NULL	NULL	0	NULL	CIS 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that CIS and superficial , noninvasive papillary TCCs strongly express E-CD .
	manualset3
124515	3	404409	13	NULL	NULL	0	NULL	noninvasive papillary TCCs 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that CIS and superficial , noninvasive papillary TCCs strongly express E-CD .
	manualset3
124516	4	404409	13	NULL	NULL	0	NULL	E-CD	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that CIS and superficial , noninvasive papillary TCCs strongly express E-CD .
	manualset3
124517	1	404410	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that HSP90-eNOS interactions were decreased in shunt lambs and that this was associated with decreased NO generation and an increase in eNOS-dependent generation of superoxide .
	manualset3
124518	2	404410	13	NULL	NULL	0	NULL	HSP90-eNOS interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that HSP90-eNOS interactions were decreased in shunt lambs and that this was associated with decreased NO generation and an increase in eNOS-dependent generation of superoxide .
	manualset3
124519	3	404410	13	NULL	NULL	0	NULL	shunt lambs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that HSP90-eNOS interactions were decreased in shunt lambs and that this was associated with decreased NO generation and an increase in eNOS-dependent generation of superoxide .
	manualset3
124520	4	404410	13	NULL	NULL	0	NULL	NO generation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that HSP90-eNOS interactions were decreased in shunt lambs and that this was associated with decreased NO generation and an increase in eNOS-dependent generation of superoxide .
	manualset3
124521	5	404410	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that HSP90-eNOS interactions were decreased in shunt lambs and that this was associated with decreased NO generation and an increase in eNOS-dependent generation of superoxide .
	manualset3
124522	6	404410	13	NULL	NULL	0	NULL	eNOS-dependent generation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that HSP90-eNOS interactions were decreased in shunt lambs and that this was associated with decreased NO generation and an increase in eNOS-dependent generation of superoxide .
	manualset3
124523	7	404410	13	NULL	NULL	0	NULL	superoxide 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that HSP90-eNOS interactions were decreased in shunt lambs and that this was associated with decreased NO generation and an increase in eNOS-dependent generation of superoxide .
	manualset3
124524	1	404411	13	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that both the cylinder rearing task and the two stages of the mHB are suitable behavioral approaches to differentiate consequences of neonatal mild and severe brain damage on executive functioning .
	manualset3
124525	2	404411	13	NULL	NULL	0	NULL	cylinder	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that both the cylinder rearing task and the two stages of the mHB are suitable behavioral approaches to differentiate consequences of neonatal mild and severe brain damage on executive functioning .
	manualset3
124526	3	404411	13	NULL	NULL	0	NULL	task 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that both the cylinder rearing task and the two stages of the mHB are suitable behavioral approaches to differentiate consequences of neonatal mild and severe brain damage on executive functioning .
	manualset3
124527	4	404411	13	NULL	NULL	0	NULL	two stages	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that both the cylinder rearing task and the two stages of the mHB are suitable behavioral approaches to differentiate consequences of neonatal mild and severe brain damage on executive functioning .
	manualset3
124528	5	404411	13	NULL	NULL	0	NULL	mHB 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that both the cylinder rearing task and the two stages of the mHB are suitable behavioral approaches to differentiate consequences of neonatal mild and severe brain damage on executive functioning .
	manualset3
124529	6	404411	13	NULL	NULL	0	NULL	behavioral approaches	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that both the cylinder rearing task and the two stages of the mHB are suitable behavioral approaches to differentiate consequences of neonatal mild and severe brain damage on executive functioning .
	manualset3
124530	7	404411	13	NULL	NULL	0	NULL	consequences	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that both the cylinder rearing task and the two stages of the mHB are suitable behavioral approaches to differentiate consequences of neonatal mild and severe brain damage on executive functioning .
	manualset3
124531	8	404411	13	NULL	NULL	0	NULL	neonatal mild brain damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that both the cylinder rearing task and the two stages of the mHB are suitable behavioral approaches to differentiate consequences of neonatal mild and severe brain damage on executive functioning .
	manualset3
124532	9	404411	13	NULL	NULL	0	NULL	neonatal severe brain damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that both the cylinder rearing task and the two stages of the mHB are suitable behavioral approaches to differentiate consequences of neonatal mild and severe brain damage on executive functioning .
	manualset3
124533	10	404411	13	NULL	NULL	0	NULL	executive functioning 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that both the cylinder rearing task and the two stages of the mHB are suitable behavioral approaches to differentiate consequences of neonatal mild and severe brain damage on executive functioning .
	manualset3
124534	1	404412	13	NULL	NULL	0	NULL	dose-response bioassay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose-response bioassay involving T ( 1 ) seedlings from several of the highest expressers of active scFv demonstrated resistance to a constant exposure of picloram at 5 x 10 ( - ) ( 8 ) M. Other approaches for increasing antibody-based herbicide resistance are discussed , as further improvements are needed before practical application of this technology .
	manualset3
124535	2	404412	13	NULL	NULL	0	NULL	T ( 1 ) seedlings	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose-response bioassay involving T ( 1 ) seedlings from several of the highest expressers of active scFv demonstrated resistance to a constant exposure of picloram at 5 x 10 ( - ) ( 8 ) M. Other approaches for increasing antibody-based herbicide resistance are discussed , as further improvements are needed before practical application of this technology .
	manualset3
124536	3	404412	13	NULL	NULL	0	NULL	highest expressers	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose-response bioassay involving T ( 1 ) seedlings from several of the highest expressers of active scFv demonstrated resistance to a constant exposure of picloram at 5 x 10 ( - ) ( 8 ) M. Other approaches for increasing antibody-based herbicide resistance are discussed , as further improvements are needed before practical application of this technology .
	manualset3
124537	4	404412	13	NULL	NULL	0	NULL	active scFv	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose-response bioassay involving T ( 1 ) seedlings from several of the highest expressers of active scFv demonstrated resistance to a constant exposure of picloram at 5 x 10 ( - ) ( 8 ) M. Other approaches for increasing antibody-based herbicide resistance are discussed , as further improvements are needed before practical application of this technology .
	manualset3
124538	5	404412	13	NULL	NULL	NULL	NULL	resistance 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A dose-response bioassay involving T ( 1 ) seedlings from several of the highest expressers of active scFv demonstrated resistance to a constant exposure of picloram at 5 x 10 ( - ) ( 8 ) M. Other approaches for increasing antibody-based herbicide resistance are discussed , as further improvements are needed before practical application of this technology .
	manualset3
124539	6	404412	13	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose-response bioassay involving T ( 1 ) seedlings from several of the highest expressers of active scFv demonstrated resistance to a constant exposure of picloram at 5 x 10 ( - ) ( 8 ) M. Other approaches for increasing antibody-based herbicide resistance are discussed , as further improvements are needed before practical application of this technology .
	manualset3
124540	7	404412	13	NULL	NULL	0	NULL	picloram 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose-response bioassay involving T ( 1 ) seedlings from several of the highest expressers of active scFv demonstrated resistance to a constant exposure of picloram at 5 x 10 ( - ) ( 8 ) M. Other approaches for increasing antibody-based herbicide resistance are discussed , as further improvements are needed before practical application of this technology .
	manualset3
124541	8	404412	13	NULL	NULL	0	NULL	5 x 10 ( - ) ( 8 ) M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose-response bioassay involving T ( 1 ) seedlings from several of the highest expressers of active scFv demonstrated resistance to a constant exposure of picloram at 5 x 10 ( - ) ( 8 ) M. Other approaches for increasing antibody-based herbicide resistance are discussed , as further improvements are needed before practical application of this technology .
	manualset3
124542	9	404412	13	NULL	NULL	0	NULL	approaches	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose-response bioassay involving T ( 1 ) seedlings from several of the highest expressers of active scFv demonstrated resistance to a constant exposure of picloram at 5 x 10 ( - ) ( 8 ) M. Other approaches for increasing antibody-based herbicide resistance are discussed , as further improvements are needed before practical application of this technology .
	manualset3
124543	10	404412	13	NULL	NULL	0	NULL	herbicide resistance 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose-response bioassay involving T ( 1 ) seedlings from several of the highest expressers of active scFv demonstrated resistance to a constant exposure of picloram at 5 x 10 ( - ) ( 8 ) M. Other approaches for increasing antibody-based herbicide resistance are discussed , as further improvements are needed before practical application of this technology .
	manualset3
124544	11	404412	13	NULL	NULL	0	NULL	improvements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose-response bioassay involving T ( 1 ) seedlings from several of the highest expressers of active scFv demonstrated resistance to a constant exposure of picloram at 5 x 10 ( - ) ( 8 ) M. Other approaches for increasing antibody-based herbicide resistance are discussed , as further improvements are needed before practical application of this technology .
	manualset3
124545	12	404412	13	NULL	NULL	0	NULL	practical application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose-response bioassay involving T ( 1 ) seedlings from several of the highest expressers of active scFv demonstrated resistance to a constant exposure of picloram at 5 x 10 ( - ) ( 8 ) M. Other approaches for increasing antibody-based herbicide resistance are discussed , as further improvements are needed before practical application of this technology .
	manualset3
124546	13	404412	13	NULL	NULL	0	NULL	technology 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose-response bioassay involving T ( 1 ) seedlings from several of the highest expressers of active scFv demonstrated resistance to a constant exposure of picloram at 5 x 10 ( - ) ( 8 ) M. Other approaches for increasing antibody-based herbicide resistance are discussed , as further improvements are needed before practical application of this technology .
	manualset3
124547	1	404413	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that eclampsia may represent the end stage of at least two very different pathophysiological pathways : one in which cerebral perfusion is low because of vasospasm and another in which cerebral perfusion is increased because of abnormal autoregulation and a failure of the normal protective mechanisms .
	manualset3
124548	2	404413	13	NULL	NULL	0	NULL	eclampsia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that eclampsia may represent the end stage of at least two very different pathophysiological pathways : one in which cerebral perfusion is low because of vasospasm and another in which cerebral perfusion is increased because of abnormal autoregulation and a failure of the normal protective mechanisms .
	manualset3
124549	3	404413	13	NULL	NULL	0	NULL	end stage 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that eclampsia may represent the end stage of at least two very different pathophysiological pathways : one in which cerebral perfusion is low because of vasospasm and another in which cerebral perfusion is increased because of abnormal autoregulation and a failure of the normal protective mechanisms .
	manualset3
124550	4	404413	13	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that eclampsia may represent the end stage of at least two very different pathophysiological pathways : one in which cerebral perfusion is low because of vasospasm and another in which cerebral perfusion is increased because of abnormal autoregulation and a failure of the normal protective mechanisms .
	manualset3
124551	5	404413	13	NULL	NULL	0	NULL	pathophysiological pathways	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that eclampsia may represent the end stage of at least two very different pathophysiological pathways : one in which cerebral perfusion is low because of vasospasm and another in which cerebral perfusion is increased because of abnormal autoregulation and a failure of the normal protective mechanisms .
	manualset3
124552	6	404413	13	NULL	NULL	0	NULL	cerebral perfusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that eclampsia may represent the end stage of at least two very different pathophysiological pathways : one in which cerebral perfusion is low because of vasospasm and another in which cerebral perfusion is increased because of abnormal autoregulation and a failure of the normal protective mechanisms .
	manualset3
124553	7	404413	13	NULL	NULL	0	NULL	vasospasm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that eclampsia may represent the end stage of at least two very different pathophysiological pathways : one in which cerebral perfusion is low because of vasospasm and another in which cerebral perfusion is increased because of abnormal autoregulation and a failure of the normal protective mechanisms .
	manualset3
124554	8	404413	13	NULL	NULL	0	NULL	cerebral perfusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that eclampsia may represent the end stage of at least two very different pathophysiological pathways : one in which cerebral perfusion is low because of vasospasm and another in which cerebral perfusion is increased because of abnormal autoregulation and a failure of the normal protective mechanisms .
	manualset3
124555	9	404413	13	NULL	NULL	0	NULL	abnormal autoregulation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that eclampsia may represent the end stage of at least two very different pathophysiological pathways : one in which cerebral perfusion is low because of vasospasm and another in which cerebral perfusion is increased because of abnormal autoregulation and a failure of the normal protective mechanisms .
	manualset3
124556	10	404413	13	NULL	NULL	0	NULL	failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that eclampsia may represent the end stage of at least two very different pathophysiological pathways : one in which cerebral perfusion is low because of vasospasm and another in which cerebral perfusion is increased because of abnormal autoregulation and a failure of the normal protective mechanisms .
	manualset3
124557	11	404413	13	NULL	NULL	0	NULL	protective mechanisms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that eclampsia may represent the end stage of at least two very different pathophysiological pathways : one in which cerebral perfusion is low because of vasospasm and another in which cerebral perfusion is increased because of abnormal autoregulation and a failure of the normal protective mechanisms .
	manualset3
124558	1	404414	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that hyperhomocysteinemia may not be a serious clinical problem among patients with epilepsy , who receive either LTG or VPA .
	manualset3
124559	2	404414	13	NULL	NULL	0	NULL	hyperhomocysteinemia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that hyperhomocysteinemia may not be a serious clinical problem among patients with epilepsy , who receive either LTG or VPA .
	manualset3
124560	3	404414	13	NULL	NULL	0	NULL	serious clinical problem	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that hyperhomocysteinemia may not be a serious clinical problem among patients with epilepsy , who receive either LTG or VPA .
	manualset3
124561	4	404414	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that hyperhomocysteinemia may not be a serious clinical problem among patients with epilepsy , who receive either LTG or VPA .
	manualset3
124562	5	404414	13	NULL	NULL	0	NULL	epilepsy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that hyperhomocysteinemia may not be a serious clinical problem among patients with epilepsy , who receive either LTG or VPA .
	manualset3
124563	6	404414	13	NULL	NULL	0	NULL	LTG	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that hyperhomocysteinemia may not be a serious clinical problem among patients with epilepsy , who receive either LTG or VPA .
	manualset3
124564	7	404414	13	NULL	NULL	0	NULL	VPA	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that hyperhomocysteinemia may not be a serious clinical problem among patients with epilepsy , who receive either LTG or VPA .
	manualset3
124565	1	404415	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that multiple mtDNA rearrangements are detectable in a considerable proportion of patients with single deletions and that mtDNA duplications do not cause any oxidative impairment .
	manualset3
124566	2	404415	13	NULL	NULL	0	NULL	mtDNA rearrangements	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that multiple mtDNA rearrangements are detectable in a considerable proportion of patients with single deletions and that mtDNA duplications do not cause any oxidative impairment .
	manualset3
124567	3	404415	13	NULL	NULL	0	NULL	proportion	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that multiple mtDNA rearrangements are detectable in a considerable proportion of patients with single deletions and that mtDNA duplications do not cause any oxidative impairment .
	manualset3
124568	4	404415	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that multiple mtDNA rearrangements are detectable in a considerable proportion of patients with single deletions and that mtDNA duplications do not cause any oxidative impairment .
	manualset3
124569	5	404415	13	NULL	NULL	0	NULL	single deletions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that multiple mtDNA rearrangements are detectable in a considerable proportion of patients with single deletions and that mtDNA duplications do not cause any oxidative impairment .
	manualset3
124570	6	404415	13	NULL	NULL	0	NULL	mtDNA duplications	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that multiple mtDNA rearrangements are detectable in a considerable proportion of patients with single deletions and that mtDNA duplications do not cause any oxidative impairment .
	manualset3
124571	7	404415	13	NULL	NULL	0	NULL	oxidative impairment 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that multiple mtDNA rearrangements are detectable in a considerable proportion of patients with single deletions and that mtDNA duplications do not cause any oxidative impairment .
	manualset3
124572	1	404416	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that single-chain HLA class I constructs can form functional class I molecules capable of presenting endogenously processed antigens .
	manualset3
124573	2	404416	13	NULL	NULL	0	NULL	single-chain HLA class I constructs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that single-chain HLA class I constructs can form functional class I molecules capable of presenting endogenously processed antigens .
	manualset3
124574	3	404416	13	NULL	NULL	0	NULL	functional class I molecules	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that single-chain HLA class I constructs can form functional class I molecules capable of presenting endogenously processed antigens .
	manualset3
124575	4	404416	13	NULL	NULL	0	NULL	antigens	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate that single-chain HLA class I constructs can form functional class I molecules capable of presenting endogenously processed antigens .
	manualset3
124576	1	404417	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate the key role of syntenin-1 in the generation of functional asymmetry in T cells and provide a novel mechanistic link between receptor activation and actin polymerization and accumulation in response to extracellular stimulation .
	manualset3
124577	2	404417	13	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate the key role of syntenin-1 in the generation of functional asymmetry in T cells and provide a novel mechanistic link between receptor activation and actin polymerization and accumulation in response to extracellular stimulation .
	manualset3
124578	3	404417	13	NULL	NULL	0	NULL	syntenin-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate the key role of syntenin-1 in the generation of functional asymmetry in T cells and provide a novel mechanistic link between receptor activation and actin polymerization and accumulation in response to extracellular stimulation .
	manualset3
124579	4	404417	13	NULL	NULL	0	NULL	generation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate the key role of syntenin-1 in the generation of functional asymmetry in T cells and provide a novel mechanistic link between receptor activation and actin polymerization and accumulation in response to extracellular stimulation .
	manualset3
124580	5	404417	13	NULL	NULL	0	NULL	functional asymmetry	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate the key role of syntenin-1 in the generation of functional asymmetry in T cells and provide a novel mechanistic link between receptor activation and actin polymerization and accumulation in response to extracellular stimulation .
	manualset3
124581	6	404417	13	NULL	NULL	0	NULL	T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate the key role of syntenin-1 in the generation of functional asymmetry in T cells and provide a novel mechanistic link between receptor activation and actin polymerization and accumulation in response to extracellular stimulation .
	manualset3
124582	7	404417	13	NULL	NULL	0	NULL	novel mechanistic link 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate the key role of syntenin-1 in the generation of functional asymmetry in T cells and provide a novel mechanistic link between receptor activation and actin polymerization and accumulation in response to extracellular stimulation .
	manualset3
124583	8	404417	13	NULL	NULL	0	NULL	receptor activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate the key role of syntenin-1 in the generation of functional asymmetry in T cells and provide a novel mechanistic link between receptor activation and actin polymerization and accumulation in response to extracellular stimulation .
	manualset3
124584	9	404417	13	NULL	NULL	0	NULL	actin polymerization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate the key role of syntenin-1 in the generation of functional asymmetry in T cells and provide a novel mechanistic link between receptor activation and actin polymerization and accumulation in response to extracellular stimulation .
	manualset3
124585	10	404417	13	NULL	NULL	0	NULL	accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate the key role of syntenin-1 in the generation of functional asymmetry in T cells and provide a novel mechanistic link between receptor activation and actin polymerization and accumulation in response to extracellular stimulation .
	manualset3
124586	11	404417	13	NULL	NULL	0	NULL	response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate the key role of syntenin-1 in the generation of functional asymmetry in T cells and provide a novel mechanistic link between receptor activation and actin polymerization and accumulation in response to extracellular stimulation .
	manualset3
124587	12	404417	13	NULL	NULL	0	NULL	extracellular stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate the key role of syntenin-1 in the generation of functional asymmetry in T cells and provide a novel mechanistic link between receptor activation and actin polymerization and accumulation in response to extracellular stimulation .
	manualset3
124588	1	404418	13	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate the need to reinterpret fibrous dysplasia of bone as a disease of cells in the osteogenic lineage , related to the effects of excess cAMP on bone cell function .
	manualset3
124589	2	404418	13	NULL	NULL	0	NULL	need	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate the need to reinterpret fibrous dysplasia of bone as a disease of cells in the osteogenic lineage , related to the effects of excess cAMP on bone cell function .
	manualset3
124590	3	404418	13	NULL	NULL	0	NULL	fibrous dysplasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate the need to reinterpret fibrous dysplasia of bone as a disease of cells in the osteogenic lineage , related to the effects of excess cAMP on bone cell function .
	manualset3
124591	4	404418	13	NULL	NULL	0	NULL	bone	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate the need to reinterpret fibrous dysplasia of bone as a disease of cells in the osteogenic lineage , related to the effects of excess cAMP on bone cell function .
	manualset3
124592	5	404418	13	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate the need to reinterpret fibrous dysplasia of bone as a disease of cells in the osteogenic lineage , related to the effects of excess cAMP on bone cell function .
	manualset3
124593	6	404418	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate the need to reinterpret fibrous dysplasia of bone as a disease of cells in the osteogenic lineage , related to the effects of excess cAMP on bone cell function .
	manualset3
124595	7	404418	13	NULL	NULL	0	NULL	osteogenic lineage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate the need to reinterpret fibrous dysplasia of bone as a disease of cells in the osteogenic lineage , related to the effects of excess cAMP on bone cell function .
	manualset3
124596	8	404418	13	NULL	NULL	0	NULL	effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate the need to reinterpret fibrous dysplasia of bone as a disease of cells in the osteogenic lineage , related to the effects of excess cAMP on bone cell function .
	manualset3
124597	9	404418	13	NULL	NULL	0	NULL	excess cAMP	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate the need to reinterpret fibrous dysplasia of bone as a disease of cells in the osteogenic lineage , related to the effects of excess cAMP on bone cell function .
	manualset3
124598	10	404418	13	NULL	NULL	0	NULL	bone cell function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicate the need to reinterpret fibrous dysplasia of bone as a disease of cells in the osteogenic lineage , related to the effects of excess cAMP on bone cell function .
	manualset3
124599	1	404419	13	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicated that by increasing the concentration of PPy ( 0-30 % ) in the composite , the average fiber diameters reduced from 239 37 nm to 191 45 nm , and the tensile modulus increased from 7.9 1.6 MPa to 50.3 3.3 MPa .
	manualset3
124600	2	404419	13	NULL	NULL	0	NULL	concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicated that by increasing the concentration of PPy ( 0-30 % ) in the composite , the average fiber diameters reduced from 239 37 nm to 191 45 nm , and the tensile modulus increased from 7.9 1.6 MPa to 50.3 3.3 MPa .
	manualset3
124601	3	404419	13	NULL	NULL	0	NULL	PPy	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicated that by increasing the concentration of PPy ( 0-30 % ) in the composite , the average fiber diameters reduced from 239 37 nm to 191 45 nm , and the tensile modulus increased from 7.9 1.6 MPa to 50.3 3.3 MPa .
	manualset3
124602	4	404419	13	NULL	NULL	0	NULL	 0-30 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicated that by increasing the concentration of PPy ( 0-30 % ) in the composite , the average fiber diameters reduced from 239 37 nm to 191 45 nm , and the tensile modulus increased from 7.9 1.6 MPa to 50.3 3.3 MPa .
	manualset3
124603	5	404419	13	NULL	NULL	0	NULL	average fiber diameters	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicated that by increasing the concentration of PPy ( 0-30 % ) in the composite , the average fiber diameters reduced from 239 37 nm to 191 45 nm , and the tensile modulus increased from 7.9 1.6 MPa to 50.3 3.3 MPa .
	manualset3
124604	6	404419	13	NULL	NULL	0	NULL	239 37 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicated that by increasing the concentration of PPy ( 0-30 % ) in the composite , the average fiber diameters reduced from 239 37 nm to 191 45 nm , and the tensile modulus increased from 7.9 1.6 MPa to 50.3 3.3 MPa .
	manualset3
124605	7	404419	13	NULL	NULL	0	NULL	191 45 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicated that by increasing the concentration of PPy ( 0-30 % ) in the composite , the average fiber diameters reduced from 239 37 nm to 191 45 nm , and the tensile modulus increased from 7.9 1.6 MPa to 50.3 3.3 MPa .
	manualset3
124606	8	404419	13	NULL	NULL	0	NULL	tensile modulus	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicated that by increasing the concentration of PPy ( 0-30 % ) in the composite , the average fiber diameters reduced from 239 37 nm to 191 45 nm , and the tensile modulus increased from 7.9 1.6 MPa to 50.3 3.3 MPa .
	manualset3
124607	9	404419	13	NULL	NULL	0	NULL	7.9 1.6 MPa 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicated that by increasing the concentration of PPy ( 0-30 % ) in the composite , the average fiber diameters reduced from 239 37 nm to 191 45 nm , and the tensile modulus increased from 7.9 1.6 MPa to 50.3 3.3 MPa .
	manualset3
124608	10	404419	13	NULL	NULL	0	NULL	50.3 3.3 MPa	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data indicated that by increasing the concentration of PPy ( 0-30 % ) in the composite , the average fiber diameters reduced from 239 37 nm to 191 45 nm , and the tensile modulus increased from 7.9 1.6 MPa to 50.3 3.3 MPa .
	manualset3
124609	1	404420	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data provide evidence that the molecular and genetic complexity of mod ( mdg4 ) is caused by a large set of individual protein isoforms with specific functions in regulating the chromatin structure of different sets of genes throughout development .
	manualset3
124610	2	404420	13	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data provide evidence that the molecular and genetic complexity of mod ( mdg4 ) is caused by a large set of individual protein isoforms with specific functions in regulating the chromatin structure of different sets of genes throughout development .
	manualset3
124611	3	404420	13	NULL	NULL	0	NULL	mod ( mdg4 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data provide evidence that the molecular and genetic complexity of mod ( mdg4 ) is caused by a large set of individual protein isoforms with specific functions in regulating the chromatin structure of different sets of genes throughout development .
	manualset3
124612	4	404420	13	NULL	NULL	0	NULL	molecular complexity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data provide evidence that the molecular and genetic complexity of mod ( mdg4 ) is caused by a large set of individual protein isoforms with specific functions in regulating the chromatin structure of different sets of genes throughout development .
	manualset3
124613	5	404420	13	NULL	NULL	0	NULL	genetic complexity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data provide evidence that the molecular and genetic complexity of mod ( mdg4 ) is caused by a large set of individual protein isoforms with specific functions in regulating the chromatin structure of different sets of genes throughout development .
	manualset3
124614	6	404420	13	NULL	NULL	0	NULL	large set 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data provide evidence that the molecular and genetic complexity of mod ( mdg4 ) is caused by a large set of individual protein isoforms with specific functions in regulating the chromatin structure of different sets of genes throughout development .
	manualset3
124615	7	404420	13	NULL	NULL	0	NULL	protein isoforms 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data provide evidence that the molecular and genetic complexity of mod ( mdg4 ) is caused by a large set of individual protein isoforms with specific functions in regulating the chromatin structure of different sets of genes throughout development .
	manualset3
124616	8	404420	13	NULL	NULL	0	NULL	specific functions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data provide evidence that the molecular and genetic complexity of mod ( mdg4 ) is caused by a large set of individual protein isoforms with specific functions in regulating the chromatin structure of different sets of genes throughout development .
	manualset3
124617	9	404420	13	NULL	NULL	0	NULL	chromatin structure	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data provide evidence that the molecular and genetic complexity of mod ( mdg4 ) is caused by a large set of individual protein isoforms with specific functions in regulating the chromatin structure of different sets of genes throughout development .
	manualset3
124618	10	404420	13	NULL	NULL	0	NULL	sets of genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data provide evidence that the molecular and genetic complexity of mod ( mdg4 ) is caused by a large set of individual protein isoforms with specific functions in regulating the chromatin structure of different sets of genes throughout development .
	manualset3
124619	11	404420	13	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data provide evidence that the molecular and genetic complexity of mod ( mdg4 ) is caused by a large set of individual protein isoforms with specific functions in regulating the chromatin structure of different sets of genes throughout development .
	manualset3
124620	1	404421	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data provided valuable information for elucidating the molecular mechanism of microbial oleaginicity and for engineering microorganisms to produce metabolites of fatty acid pathway .
	manualset3
124621	2	404421	13	NULL	NULL	0	NULL	information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data provided valuable information for elucidating the molecular mechanism of microbial oleaginicity and for engineering microorganisms to produce metabolites of fatty acid pathway .
	manualset3
124622	3	404421	13	NULL	NULL	0	NULL	molecular mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data provided valuable information for elucidating the molecular mechanism of microbial oleaginicity and for engineering microorganisms to produce metabolites of fatty acid pathway .
	manualset3
124623	4	404421	13	NULL	NULL	0	NULL	microbial oleaginicity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data provided valuable information for elucidating the molecular mechanism of microbial oleaginicity and for engineering microorganisms to produce metabolites of fatty acid pathway .
	manualset3
124624	5	404421	13	NULL	NULL	0	NULL	engineering 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data provided valuable information for elucidating the molecular mechanism of microbial oleaginicity and for engineering microorganisms to produce metabolites of fatty acid pathway .
	manualset3
124625	6	404421	13	NULL	NULL	0	NULL	microorganisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data provided valuable information for elucidating the molecular mechanism of microbial oleaginicity and for engineering microorganisms to produce metabolites of fatty acid pathway .
	manualset3
124626	7	404421	13	NULL	NULL	0	NULL	metabolites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data provided valuable information for elucidating the molecular mechanism of microbial oleaginicity and for engineering microorganisms to produce metabolites of fatty acid pathway .
	manualset3
124627	8	404421	13	NULL	NULL	0	NULL	fatty acid pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data provided valuable information for elucidating the molecular mechanism of microbial oleaginicity and for engineering microorganisms to produce metabolites of fatty acid pathway .
	manualset3
124628	1	404422	13	NULL	NULL	NULL	NULL	dose	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A dose ( 0.25 microg/ml ) of filipin for 30 min produced a similar effect ( +111 % , P & lt ; 0.05 ) .
	manualset3
124629	2	404422	13	NULL	NULL	0	NULL	0.25 microg/ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose ( 0.25 microg/ml ) of filipin for 30 min produced a similar effect ( +111 % , P & lt ; 0.05 ) .
	manualset3
124630	3	404422	13	NULL	NULL	0	NULL	filipin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose ( 0.25 microg/ml ) of filipin for 30 min produced a similar effect ( +111 % , P & lt ; 0.05 ) .
	manualset3
124631	4	404422	13	NULL	NULL	NULL	NULL	30 min	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A dose ( 0.25 microg/ml ) of filipin for 30 min produced a similar effect ( +111 % , P & lt ; 0.05 ) .
	manualset3
124632	5	404422	13	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose ( 0.25 microg/ml ) of filipin for 30 min produced a similar effect ( +111 % , P & lt ; 0.05 ) .
	manualset3
124633	6	404422	13	NULL	NULL	0	NULL	 +111 % , P & lt ; 0.05 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose ( 0.25 microg/ml ) of filipin for 30 min produced a similar effect ( +111 % , P & lt ; 0.05 ) .
	manualset3
124634	1	404423	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data raise the possibility that gender differences in adiponectin may be lost in diabetes .
	manualset3
124635	2	404423	13	NULL	NULL	0	NULL	possibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data raise the possibility that gender differences in adiponectin may be lost in diabetes .
	manualset3
124636	3	404423	13	NULL	NULL	0	NULL	gender differences 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data raise the possibility that gender differences in adiponectin may be lost in diabetes .
	manualset3
124637	4	404423	13	NULL	NULL	0	NULL	adiponectin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data raise the possibility that gender differences in adiponectin may be lost in diabetes .
	manualset3
124638	5	404423	13	NULL	NULL	0	NULL	diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data raise the possibility that gender differences in adiponectin may be lost in diabetes .
	manualset3
124639	1	404424	13	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show a decreased Foxp3 expression and an increased ROR gamma t expression in COPD patients and normal smokers that parallels the aggravation of the disease .
	manualset3
124640	2	404424	13	NULL	NULL	0	NULL	Foxp3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show a decreased Foxp3 expression and an increased ROR gamma t expression in COPD patients and normal smokers that parallels the aggravation of the disease .
	manualset3
124641	3	404424	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show a decreased Foxp3 expression and an increased ROR gamma t expression in COPD patients and normal smokers that parallels the aggravation of the disease .
	manualset3
124642	4	404424	13	NULL	NULL	0	NULL	ROR gamma t 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show a decreased Foxp3 expression and an increased ROR gamma t expression in COPD patients and normal smokers that parallels the aggravation of the disease .
	manualset3
124643	5	404424	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show a decreased Foxp3 expression and an increased ROR gamma t expression in COPD patients and normal smokers that parallels the aggravation of the disease .
	manualset3
124644	6	404424	13	NULL	NULL	0	NULL	COPD patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show a decreased Foxp3 expression and an increased ROR gamma t expression in COPD patients and normal smokers that parallels the aggravation of the disease .
	manualset3
124645	7	404424	13	NULL	NULL	0	NULL	smokers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show a decreased Foxp3 expression and an increased ROR gamma t expression in COPD patients and normal smokers that parallels the aggravation of the disease .
	manualset3
124646	8	404424	13	NULL	NULL	0	NULL	aggravation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show a decreased Foxp3 expression and an increased ROR gamma t expression in COPD patients and normal smokers that parallels the aggravation of the disease .
	manualset3
124647	9	404424	13	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show a decreased Foxp3 expression and an increased ROR gamma t expression in COPD patients and normal smokers that parallels the aggravation of the disease .
	manualset3
124648	1	404425	13	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that endocytosis of PEGylated probes and drugs enhances both cancer imaging and anticancer efficacy , indicating that endocytic receptors are superior targets for the design of cancer imaging probes and immunoliposomal drugs .
	manualset3
124649	2	404425	13	NULL	NULL	0	NULL	endocytosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that endocytosis of PEGylated probes and drugs enhances both cancer imaging and anticancer efficacy , indicating that endocytic receptors are superior targets for the design of cancer imaging probes and immunoliposomal drugs .
	manualset3
124650	3	404425	13	NULL	NULL	0	NULL	PEGylated probes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that endocytosis of PEGylated probes and drugs enhances both cancer imaging and anticancer efficacy , indicating that endocytic receptors are superior targets for the design of cancer imaging probes and immunoliposomal drugs .
	manualset3
124651	4	404425	13	NULL	NULL	0	NULL	drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that endocytosis of PEGylated probes and drugs enhances both cancer imaging and anticancer efficacy , indicating that endocytic receptors are superior targets for the design of cancer imaging probes and immunoliposomal drugs .
	manualset3
124652	5	404425	13	NULL	NULL	0	NULL	cancer imaging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that endocytosis of PEGylated probes and drugs enhances both cancer imaging and anticancer efficacy , indicating that endocytic receptors are superior targets for the design of cancer imaging probes and immunoliposomal drugs .
	manualset3
124653	6	404425	13	NULL	NULL	0	NULL	anticancer efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that endocytosis of PEGylated probes and drugs enhances both cancer imaging and anticancer efficacy , indicating that endocytic receptors are superior targets for the design of cancer imaging probes and immunoliposomal drugs .
	manualset3
124654	7	404425	13	NULL	NULL	0	NULL	endocytic receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that endocytosis of PEGylated probes and drugs enhances both cancer imaging and anticancer efficacy , indicating that endocytic receptors are superior targets for the design of cancer imaging probes and immunoliposomal drugs .
	manualset3
124655	8	404425	13	NULL	NULL	0	NULL	targets	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that endocytosis of PEGylated probes and drugs enhances both cancer imaging and anticancer efficacy , indicating that endocytic receptors are superior targets for the design of cancer imaging probes and immunoliposomal drugs .
	manualset3
124656	9	404425	13	NULL	NULL	0	NULL	design	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that endocytosis of PEGylated probes and drugs enhances both cancer imaging and anticancer efficacy , indicating that endocytic receptors are superior targets for the design of cancer imaging probes and immunoliposomal drugs .
	manualset3
124657	10	404425	13	NULL	NULL	0	NULL	cancer imaging probes 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that endocytosis of PEGylated probes and drugs enhances both cancer imaging and anticancer efficacy , indicating that endocytic receptors are superior targets for the design of cancer imaging probes and immunoliposomal drugs .
	manualset3
124658	11	404425	13	NULL	NULL	0	NULL	immunoliposomal drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that endocytosis of PEGylated probes and drugs enhances both cancer imaging and anticancer efficacy , indicating that endocytic receptors are superior targets for the design of cancer imaging probes and immunoliposomal drugs .
	manualset3
124659	1	404426	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that morphine is able to exert a significant enhancement of the response of beta 2-adrenergic receptors to isoproterenol in human mononuclear leukocytes .
	manualset3
124660	2	404426	13	NULL	NULL	0	NULL	morphine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that morphine is able to exert a significant enhancement of the response of beta 2-adrenergic receptors to isoproterenol in human mononuclear leukocytes .
	manualset3
124661	3	404426	13	NULL	NULL	0	NULL	enhancement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that morphine is able to exert a significant enhancement of the response of beta 2-adrenergic receptors to isoproterenol in human mononuclear leukocytes .
	manualset3
124662	4	404426	13	NULL	NULL	0	NULL	response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that morphine is able to exert a significant enhancement of the response of beta 2-adrenergic receptors to isoproterenol in human mononuclear leukocytes .
	manualset3
124663	5	404426	13	NULL	NULL	0	NULL	beta 2-adrenergic receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that morphine is able to exert a significant enhancement of the response of beta 2-adrenergic receptors to isoproterenol in human mononuclear leukocytes .
	manualset3
124664	6	404426	13	NULL	NULL	0	NULL	isoproterenol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that morphine is able to exert a significant enhancement of the response of beta 2-adrenergic receptors to isoproterenol in human mononuclear leukocytes .
	manualset3
124665	7	404426	13	NULL	NULL	0	NULL	human mononuclear leukocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that morphine is able to exert a significant enhancement of the response of beta 2-adrenergic receptors to isoproterenol in human mononuclear leukocytes .
	manualset3
124666	1	404427	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that neuronally expressed S1P receptors play a significant role in regulating nociceptor function and that S1P/S1P signaling may be a key player in the onset of thermal hypersensitivity and hyperalgesia associated with inflammation .
	manualset3
124667	2	404427	13	NULL	NULL	0	NULL	S1P receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that neuronally expressed S1P receptors play a significant role in regulating nociceptor function and that S1P/S1P signaling may be a key player in the onset of thermal hypersensitivity and hyperalgesia associated with inflammation .
	manualset3
124668	3	404427	13	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that neuronally expressed S1P receptors play a significant role in regulating nociceptor function and that S1P/S1P signaling may be a key player in the onset of thermal hypersensitivity and hyperalgesia associated with inflammation .
	manualset3
124669	4	404427	13	NULL	NULL	0	NULL	nociceptor function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that neuronally expressed S1P receptors play a significant role in regulating nociceptor function and that S1P/S1P signaling may be a key player in the onset of thermal hypersensitivity and hyperalgesia associated with inflammation .
	manualset3
124670	5	404427	13	NULL	NULL	0	NULL	 S1P/S1P signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that neuronally expressed S1P receptors play a significant role in regulating nociceptor function and that S1P/S1P signaling may be a key player in the onset of thermal hypersensitivity and hyperalgesia associated with inflammation .
	manualset3
124671	6	404427	13	NULL	NULL	0	NULL	key player	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that neuronally expressed S1P receptors play a significant role in regulating nociceptor function and that S1P/S1P signaling may be a key player in the onset of thermal hypersensitivity and hyperalgesia associated with inflammation .
	manualset3
124672	7	404427	13	NULL	NULL	0	NULL	onset of thermal hypersensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that neuronally expressed S1P receptors play a significant role in regulating nociceptor function and that S1P/S1P signaling may be a key player in the onset of thermal hypersensitivity and hyperalgesia associated with inflammation .
	manualset3
124673	8	404427	13	NULL	NULL	0	NULL	hyperalgesia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that neuronally expressed S1P receptors play a significant role in regulating nociceptor function and that S1P/S1P signaling may be a key player in the onset of thermal hypersensitivity and hyperalgesia associated with inflammation .
	manualset3
124674	9	404427	13	NULL	NULL	0	NULL	inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that neuronally expressed S1P receptors play a significant role in regulating nociceptor function and that S1P/S1P signaling may be a key player in the onset of thermal hypersensitivity and hyperalgesia associated with inflammation .
	manualset3
124675	1	404428	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that the delay between onset of symptoms and diagnosis is far greater than previously supposed and that most babies detected by our screening program already had symptoms that warranted treatment at the time of their diagnosis .
	manualset3
124676	2	404428	13	NULL	NULL	0	NULL	delay 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that the delay between onset of symptoms and diagnosis is far greater than previously supposed and that most babies detected by our screening program already had symptoms that warranted treatment at the time of their diagnosis .
	manualset3
124677	3	404428	13	NULL	NULL	0	NULL	onset of symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that the delay between onset of symptoms and diagnosis is far greater than previously supposed and that most babies detected by our screening program already had symptoms that warranted treatment at the time of their diagnosis .
	manualset3
124678	4	404428	13	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that the delay between onset of symptoms and diagnosis is far greater than previously supposed and that most babies detected by our screening program already had symptoms that warranted treatment at the time of their diagnosis .
	manualset3
124679	5	404428	13	NULL	NULL	0	NULL	babies 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that the delay between onset of symptoms and diagnosis is far greater than previously supposed and that most babies detected by our screening program already had symptoms that warranted treatment at the time of their diagnosis .
	manualset3
124680	6	404428	13	NULL	NULL	0	NULL	screening program	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that the delay between onset of symptoms and diagnosis is far greater than previously supposed and that most babies detected by our screening program already had symptoms that warranted treatment at the time of their diagnosis .
	manualset3
124681	7	404428	13	NULL	NULL	0	NULL	symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that the delay between onset of symptoms and diagnosis is far greater than previously supposed and that most babies detected by our screening program already had symptoms that warranted treatment at the time of their diagnosis .
	manualset3
124682	8	404428	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that the delay between onset of symptoms and diagnosis is far greater than previously supposed and that most babies detected by our screening program already had symptoms that warranted treatment at the time of their diagnosis .
	manualset3
124683	9	404428	13	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that the delay between onset of symptoms and diagnosis is far greater than previously supposed and that most babies detected by our screening program already had symptoms that warranted treatment at the time of their diagnosis .
	manualset3
124684	10	404428	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data show that the delay between onset of symptoms and diagnosis is far greater than previously supposed and that most babies detected by our screening program already had symptoms that warranted treatment at the time of their diagnosis .
	manualset3
124685	1	404429	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest a possible direct relationship between fasting insulinemia and blood pressure , especially in obese patients or patients with impaired glucose metabolism , and that increased blood pressure per se is not an insulin resistant state .
	manualset3
124686	2	404429	13	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest a possible direct relationship between fasting insulinemia and blood pressure , especially in obese patients or patients with impaired glucose metabolism , and that increased blood pressure per se is not an insulin resistant state .
	manualset3
124687	3	404429	13	NULL	NULL	0	NULL	insulinemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest a possible direct relationship between fasting insulinemia and blood pressure , especially in obese patients or patients with impaired glucose metabolism , and that increased blood pressure per se is not an insulin resistant state .
	manualset3
124688	4	404429	13	NULL	NULL	0	NULL	blood pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest a possible direct relationship between fasting insulinemia and blood pressure , especially in obese patients or patients with impaired glucose metabolism , and that increased blood pressure per se is not an insulin resistant state .
	manualset3
124689	5	404429	13	NULL	NULL	0	NULL	obese patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest a possible direct relationship between fasting insulinemia and blood pressure , especially in obese patients or patients with impaired glucose metabolism , and that increased blood pressure per se is not an insulin resistant state .
	manualset3
124690	6	404429	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest a possible direct relationship between fasting insulinemia and blood pressure , especially in obese patients or patients with impaired glucose metabolism , and that increased blood pressure per se is not an insulin resistant state .
	manualset3
124691	7	404429	13	NULL	NULL	0	NULL	glucose metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest a possible direct relationship between fasting insulinemia and blood pressure , especially in obese patients or patients with impaired glucose metabolism , and that increased blood pressure per se is not an insulin resistant state .
	manualset3
124692	8	404429	13	NULL	NULL	NULL	NULL	blood pressure per se	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our data suggest a possible direct relationship between fasting insulinemia and blood pressure , especially in obese patients or patients with impaired glucose metabolism , and that increased blood pressure per se is not an insulin resistant state .
	manualset3
124693	9	404429	13	NULL	NULL	0	NULL	insulin resistant state	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest a possible direct relationship between fasting insulinemia and blood pressure , especially in obese patients or patients with impaired glucose metabolism , and that increased blood pressure per se is not an insulin resistant state .
	manualset3
124694	1	404430	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest a re-evaluation of the contribution of `` null '' alleles to XPD disorders and highlight the potential of combinations of recessive alleles to affect both normal and pathological phenotypic plasticity in mammals .
	manualset3
124695	2	404430	13	NULL	NULL	0	NULL	re-evaluation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest a re-evaluation of the contribution of `` null '' alleles to XPD disorders and highlight the potential of combinations of recessive alleles to affect both normal and pathological phenotypic plasticity in mammals .
	manualset3
124696	3	404430	13	NULL	NULL	0	NULL	contribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest a re-evaluation of the contribution of `` null '' alleles to XPD disorders and highlight the potential of combinations of recessive alleles to affect both normal and pathological phenotypic plasticity in mammals .
	manualset3
124697	4	404430	13	NULL	NULL	0	NULL	`` null '' alleles 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest a re-evaluation of the contribution of `` null '' alleles to XPD disorders and highlight the potential of combinations of recessive alleles to affect both normal and pathological phenotypic plasticity in mammals .
	manualset3
124699	5	404430	13	NULL	NULL	0	NULL	XPD disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest a re-evaluation of the contribution of `` null '' alleles to XPD disorders and highlight the potential of combinations of recessive alleles to affect both normal and pathological phenotypic plasticity in mammals .
	manualset3
124700	6	404430	13	NULL	NULL	0	NULL	highlight 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest a re-evaluation of the contribution of `` null '' alleles to XPD disorders and highlight the potential of combinations of recessive alleles to affect both normal and pathological phenotypic plasticity in mammals .
	manualset3
124701	7	404430	13	NULL	NULL	0	NULL	potential 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest a re-evaluation of the contribution of `` null '' alleles to XPD disorders and highlight the potential of combinations of recessive alleles to affect both normal and pathological phenotypic plasticity in mammals .
	manualset3
124702	8	404430	13	NULL	NULL	0	NULL	combinations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest a re-evaluation of the contribution of `` null '' alleles to XPD disorders and highlight the potential of combinations of recessive alleles to affect both normal and pathological phenotypic plasticity in mammals .
	manualset3
124703	9	404430	13	NULL	NULL	0	NULL	recessive alleles	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest a re-evaluation of the contribution of `` null '' alleles to XPD disorders and highlight the potential of combinations of recessive alleles to affect both normal and pathological phenotypic plasticity in mammals .
	manualset3
124704	10	404430	13	NULL	NULL	NULL	NULL	normal phenotypic plasticity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our data suggest a re-evaluation of the contribution of `` null '' alleles to XPD disorders and highlight the potential of combinations of recessive alleles to affect both normal and pathological phenotypic plasticity in mammals .
	manualset3
124705	11	404430	13	NULL	NULL	NULL	NULL	pathological phenotypic plasticity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our data suggest a re-evaluation of the contribution of `` null '' alleles to XPD disorders and highlight the potential of combinations of recessive alleles to affect both normal and pathological phenotypic plasticity in mammals .
	manualset3
124706	12	404430	13	NULL	NULL	0	NULL	mammals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest a re-evaluation of the contribution of `` null '' alleles to XPD disorders and highlight the potential of combinations of recessive alleles to affect both normal and pathological phenotypic plasticity in mammals .
	manualset3
124707	1	404431	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that EXL1 is part of a regulatory pathway that controls growth and development when C and energy supply is poor .
	manualset3
124708	2	404431	13	NULL	NULL	0	NULL	EXL1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that EXL1 is part of a regulatory pathway that controls growth and development when C and energy supply is poor .
	manualset3
124709	3	404431	13	NULL	NULL	0	NULL	regulatory pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that EXL1 is part of a regulatory pathway that controls growth and development when C and energy supply is poor .
	manualset3
124710	4	404431	13	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that EXL1 is part of a regulatory pathway that controls growth and development when C and energy supply is poor .
	manualset3
124711	5	404431	13	NULL	NULL	0	NULL	development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that EXL1 is part of a regulatory pathway that controls growth and development when C and energy supply is poor .
	manualset3
124712	6	404431	13	NULL	NULL	0	NULL	C 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that EXL1 is part of a regulatory pathway that controls growth and development when C and energy supply is poor .
	manualset3
124713	7	404431	13	NULL	NULL	0	NULL	energy supply 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that EXL1 is part of a regulatory pathway that controls growth and development when C and energy supply is poor .
	manualset3
124714	1	404432	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that alterations in the expression of GABAA receptor subunits in the AD hippocampus differ between specific receptor subunits with the amount of beta2 mRNA being relatively well-preserved , while beta3 mRNA levels were decreased .
	manualset3
124715	2	404432	13	NULL	NULL	0	NULL	alterations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that alterations in the expression of GABAA receptor subunits in the AD hippocampus differ between specific receptor subunits with the amount of beta2 mRNA being relatively well-preserved , while beta3 mRNA levels were decreased .
	manualset3
124716	3	404432	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that alterations in the expression of GABAA receptor subunits in the AD hippocampus differ between specific receptor subunits with the amount of beta2 mRNA being relatively well-preserved , while beta3 mRNA levels were decreased .
	manualset3
124717	4	404432	13	NULL	NULL	0	NULL	GABAA receptor subunits	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that alterations in the expression of GABAA receptor subunits in the AD hippocampus differ between specific receptor subunits with the amount of beta2 mRNA being relatively well-preserved , while beta3 mRNA levels were decreased .
	manualset3
124718	5	404432	13	NULL	NULL	0	NULL	AD hippocampus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that alterations in the expression of GABAA receptor subunits in the AD hippocampus differ between specific receptor subunits with the amount of beta2 mRNA being relatively well-preserved , while beta3 mRNA levels were decreased .
	manualset3
124719	6	404432	13	NULL	NULL	0	NULL	 specific receptor subunits	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that alterations in the expression of GABAA receptor subunits in the AD hippocampus differ between specific receptor subunits with the amount of beta2 mRNA being relatively well-preserved , while beta3 mRNA levels were decreased .
	manualset3
124720	7	404432	13	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that alterations in the expression of GABAA receptor subunits in the AD hippocampus differ between specific receptor subunits with the amount of beta2 mRNA being relatively well-preserved , while beta3 mRNA levels were decreased .
	manualset3
124721	8	404432	13	NULL	NULL	0	NULL	beta2 mRNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that alterations in the expression of GABAA receptor subunits in the AD hippocampus differ between specific receptor subunits with the amount of beta2 mRNA being relatively well-preserved , while beta3 mRNA levels were decreased .
	manualset3
124722	9	404432	13	NULL	NULL	0	NULL	beta3 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that alterations in the expression of GABAA receptor subunits in the AD hippocampus differ between specific receptor subunits with the amount of beta2 mRNA being relatively well-preserved , while beta3 mRNA levels were decreased .
	manualset3
124723	10	404432	13	NULL	NULL	0	NULL	levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that alterations in the expression of GABAA receptor subunits in the AD hippocampus differ between specific receptor subunits with the amount of beta2 mRNA being relatively well-preserved , while beta3 mRNA levels were decreased .
	manualset3
124724	1	404433	13	NULL	NULL	0	NULL	dose - dependent association	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose - and time-dependent association among AMPA receptors , the focal adhesion kinase pp125FAK , the phosphatidylinositol-3 kinase and paxillin was found .
	manualset3
124725	2	404433	13	NULL	NULL	0	NULL	time-dependent association 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose - and time-dependent association among AMPA receptors , the focal adhesion kinase pp125FAK , the phosphatidylinositol-3 kinase and paxillin was found .
	manualset3
124726	3	404433	13	NULL	NULL	0	NULL	AMPA receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose - and time-dependent association among AMPA receptors , the focal adhesion kinase pp125FAK , the phosphatidylinositol-3 kinase and paxillin was found .
	manualset3
124727	4	404433	13	NULL	NULL	0	NULL	focal adhesion kinase pp125FAK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose - and time-dependent association among AMPA receptors , the focal adhesion kinase pp125FAK , the phosphatidylinositol-3 kinase and paxillin was found .
	manualset3
124728	5	404433	13	NULL	NULL	0	NULL	phosphatidylinositol-3 kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose - and time-dependent association among AMPA receptors , the focal adhesion kinase pp125FAK , the phosphatidylinositol-3 kinase and paxillin was found .
	manualset3
124729	6	404433	13	NULL	NULL	0	NULL	paxillin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose - and time-dependent association among AMPA receptors , the focal adhesion kinase pp125FAK , the phosphatidylinositol-3 kinase and paxillin was found .
	manualset3
124730	1	404434	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that estradiol in vivo and in vitro interferes with the effect of GTP on striatal D-2 DA receptors .
	manualset3
124731	2	404434	13	NULL	NULL	0	NULL	estradiol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that estradiol in vivo and in vitro interferes with the effect of GTP on striatal D-2 DA receptors .
	manualset3
124732	3	404434	13	NULL	NULL	0	NULL	effect of GTP 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that estradiol in vivo and in vitro interferes with the effect of GTP on striatal D-2 DA receptors .
	manualset3
124733	4	404434	13	NULL	NULL	0	NULL	striatal D-2 DA receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that estradiol in vivo and in vitro interferes with the effect of GTP on striatal D-2 DA receptors .
	manualset3
124734	1	404435	13	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that genistein has direct genomic effects on the vascular wall that are unrelated to its known actions , leading to increased eNOS expression and NO synthesis , thereby improving hypertension .
	manualset3
124735	2	404435	13	NULL	NULL	0	NULL	genistein	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that genistein has direct genomic effects on the vascular wall that are unrelated to its known actions , leading to increased eNOS expression and NO synthesis , thereby improving hypertension .
	manualset3
124742	3	404435	13	NULL	NULL	0	NULL	genomic effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that genistein has direct genomic effects on the vascular wall that are unrelated to its known actions , leading to increased eNOS expression and NO synthesis , thereby improving hypertension .
	manualset3
124743	4	404435	13	NULL	NULL	0	NULL	vascular wall 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that genistein has direct genomic effects on the vascular wall that are unrelated to its known actions , leading to increased eNOS expression and NO synthesis , thereby improving hypertension .
	manualset3
124744	5	404435	13	NULL	NULL	0	NULL	actions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that genistein has direct genomic effects on the vascular wall that are unrelated to its known actions , leading to increased eNOS expression and NO synthesis , thereby improving hypertension .
	manualset3
124745	6	404435	13	NULL	NULL	0	NULL	eNOS	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that genistein has direct genomic effects on the vascular wall that are unrelated to its known actions , leading to increased eNOS expression and NO synthesis , thereby improving hypertension .
	manualset3
124746	7	404435	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that genistein has direct genomic effects on the vascular wall that are unrelated to its known actions , leading to increased eNOS expression and NO synthesis , thereby improving hypertension .
	manualset3
124747	8	404435	13	NULL	NULL	0	NULL	NO synthesis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that genistein has direct genomic effects on the vascular wall that are unrelated to its known actions , leading to increased eNOS expression and NO synthesis , thereby improving hypertension .
	manualset3
124749	9	404435	13	NULL	NULL	0	NULL	hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that genistein has direct genomic effects on the vascular wall that are unrelated to its known actions , leading to increased eNOS expression and NO synthesis , thereby improving hypertension .
	manualset3
124750	1	404436	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that none of these LMP2 or LMP7 polymorphisms are independently associated with IDDM susceptibility , in contrast to what has been previously reported by others .
	manualset3
124751	2	404436	13	NULL	NULL	0	NULL	LMP2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that none of these LMP2 or LMP7 polymorphisms are independently associated with IDDM susceptibility , in contrast to what has been previously reported by others .
	manualset3
124752	3	404436	13	NULL	NULL	0	NULL	LMP7	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that none of these LMP2 or LMP7 polymorphisms are independently associated with IDDM susceptibility , in contrast to what has been previously reported by others .
	manualset3
124753	4	404436	13	NULL	NULL	0	NULL	polymorphisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that none of these LMP2 or LMP7 polymorphisms are independently associated with IDDM susceptibility , in contrast to what has been previously reported by others .
	manualset3
124754	5	404436	13	NULL	NULL	0	NULL	IDDM susceptibility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that none of these LMP2 or LMP7 polymorphisms are independently associated with IDDM susceptibility , in contrast to what has been previously reported by others .
	manualset3
124755	6	404436	13	NULL	NULL	0	NULL	contrast	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that none of these LMP2 or LMP7 polymorphisms are independently associated with IDDM susceptibility , in contrast to what has been previously reported by others .
	manualset3
124756	7	404436	13	NULL	NULL	0	NULL	others	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that none of these LMP2 or LMP7 polymorphisms are independently associated with IDDM susceptibility , in contrast to what has been previously reported by others .
	manualset3
124757	1	404437	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that p21 does not discriminate in vitro `` repair '' and `` replication '' DNA synthesis based on template length but does act preferentially on polymerization which encounters obstacles to progress .
	manualset3
124758	2	404437	13	NULL	NULL	0	NULL	p21	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that p21 does not discriminate in vitro `` repair '' and `` replication '' DNA synthesis based on template length but does act preferentially on polymerization which encounters obstacles to progress .
	manualset3
124760	3	404437	13	NULL	NULL	0	NULL	`` repair ''	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that p21 does not discriminate in vitro `` repair '' and `` replication '' DNA synthesis based on template length but does act preferentially on polymerization which encounters obstacles to progress .
	manualset3
124761	4	404437	13	NULL	NULL	0	NULL	`` replication '' 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that p21 does not discriminate in vitro `` repair '' and `` replication '' DNA synthesis based on template length but does act preferentially on polymerization which encounters obstacles to progress .
	manualset3
124762	5	404437	13	NULL	NULL	0	NULL	DNA synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that p21 does not discriminate in vitro `` repair '' and `` replication '' DNA synthesis based on template length but does act preferentially on polymerization which encounters obstacles to progress .
	manualset3
124763	6	404437	13	NULL	NULL	0	NULL	template length	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that p21 does not discriminate in vitro `` repair '' and `` replication '' DNA synthesis based on template length but does act preferentially on polymerization which encounters obstacles to progress .
	manualset3
124765	8	404437	13	NULL	NULL	0	NULL	polymerization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that p21 does not discriminate in vitro `` repair '' and `` replication '' DNA synthesis based on template length but does act preferentially on polymerization which encounters obstacles to progress .
	manualset3
124766	9	404437	13	NULL	NULL	0	NULL	obstacles 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggest that p21 does not discriminate in vitro `` repair '' and `` replication '' DNA synthesis based on template length but does act preferentially on polymerization which encounters obstacles to progress .
	manualset3
124767	1	404438	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggested that E2 could regulate the immunoreaction in the nicotine-induced inflammatory process possibly through classic intercellular ER , whereas Te had no significant effect in this process .
	manualset3
124769	2	404438	13	NULL	NULL	0	NULL	E2 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggested that E2 could regulate the immunoreaction in the nicotine-induced inflammatory process possibly through classic intercellular ER , whereas Te had no significant effect in this process .
	manualset3
124771	3	404438	13	NULL	NULL	0	NULL	immunoreaction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggested that E2 could regulate the immunoreaction in the nicotine-induced inflammatory process possibly through classic intercellular ER , whereas Te had no significant effect in this process .
	manualset3
124772	4	404438	13	NULL	NULL	0	NULL	nicotine-induced inflammatory process	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggested that E2 could regulate the immunoreaction in the nicotine-induced inflammatory process possibly through classic intercellular ER , whereas Te had no significant effect in this process .
	manualset3
124773	5	404438	13	NULL	NULL	0	NULL	classic intercellular ER	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggested that E2 could regulate the immunoreaction in the nicotine-induced inflammatory process possibly through classic intercellular ER , whereas Te had no significant effect in this process .
	manualset3
124774	6	404438	13	NULL	NULL	0	NULL	Te	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggested that E2 could regulate the immunoreaction in the nicotine-induced inflammatory process possibly through classic intercellular ER , whereas Te had no significant effect in this process .
	manualset3
124775	7	404438	13	NULL	NULL	0	NULL	effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggested that E2 could regulate the immunoreaction in the nicotine-induced inflammatory process possibly through classic intercellular ER , whereas Te had no significant effect in this process .
	manualset3
124776	8	404438	13	NULL	NULL	0	NULL	process	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data suggested that E2 could regulate the immunoreaction in the nicotine-induced inflammatory process possibly through classic intercellular ER , whereas Te had no significant effect in this process .
	manualset3
124777	1	404439	13	NULL	NULL	0	NULL	implications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our finding may also have implications for the use of aggregate variables in epidemiology to control for unmeasured confounding .
	manualset3
124778	2	404439	13	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our finding may also have implications for the use of aggregate variables in epidemiology to control for unmeasured confounding .
	manualset3
124779	3	404439	13	NULL	NULL	0	NULL	aggregate variables	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our finding may also have implications for the use of aggregate variables in epidemiology to control for unmeasured confounding .
	manualset3
124780	4	404439	13	NULL	NULL	0	NULL	epidemiology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Our finding may also have implications for the use of aggregate variables in epidemiology to control for unmeasured confounding .
	manualset3
128809	5	404439	13	NULL	NULL	0	NULL	confounding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our finding may also have implications for the use of aggregate variables in epidemiology to control for unmeasured confounding .
	manualset3
124781	1	404440	13	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings do not support a role for gastric cell lysosomes in histamine-induced gastric mucosal injury .
	manualset3
124782	2	404440	13	NULL	NULL	0	NULL	role 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings do not support a role for gastric cell lysosomes in histamine-induced gastric mucosal injury .
	manualset3
124783	3	404440	13	NULL	NULL	0	NULL	gastric cell lysosomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings do not support a role for gastric cell lysosomes in histamine-induced gastric mucosal injury .
	manualset3
124785	4	404440	13	NULL	NULL	0	NULL	gastric mucosal injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings do not support a role for gastric cell lysosomes in histamine-induced gastric mucosal injury .
	manualset3
124787	1	404441	13	NULL	NULL	0	NULL	findings	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings implicate these candidate genes in the etiology of colon and rectal cancer and provide information on how these genes operate with other genes in the pathway .
	manualset3
124789	2	404441	13	NULL	NULL	0	NULL	candidate genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings implicate these candidate genes in the etiology of colon and rectal cancer and provide information on how these genes operate with other genes in the pathway .
	manualset3
124790	3	404441	13	NULL	NULL	0	NULL	etiology of colon	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings implicate these candidate genes in the etiology of colon and rectal cancer and provide information on how these genes operate with other genes in the pathway .
	manualset3
124792	4	404441	13	NULL	NULL	0	NULL	rectal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings implicate these candidate genes in the etiology of colon and rectal cancer and provide information on how these genes operate with other genes in the pathway .
	manualset3
124794	5	404441	13	NULL	NULL	0	NULL	information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings implicate these candidate genes in the etiology of colon and rectal cancer and provide information on how these genes operate with other genes in the pathway .
	manualset3
124795	6	404441	13	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings implicate these candidate genes in the etiology of colon and rectal cancer and provide information on how these genes operate with other genes in the pathway .
	manualset3
124796	7	404441	13	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings implicate these candidate genes in the etiology of colon and rectal cancer and provide information on how these genes operate with other genes in the pathway .
	manualset3
124797	8	404441	13	NULL	NULL	0	NULL	pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings implicate these candidate genes in the etiology of colon and rectal cancer and provide information on how these genes operate with other genes in the pathway .
	manualset3
124798	1	404442	13	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings indicate not only that this case-finding approach is effective in identifying FH patients who otherwise would not have been identified but also that the vast majority of these patients seek treatment and are successfully started on cholesterol-lowering therapy to reduce their risk of premature cardiovascular disease .
	manualset3
124799	2	404442	13	NULL	NULL	0	NULL	case-finding approach	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings indicate not only that this case-finding approach is effective in identifying FH patients who otherwise would not have been identified but also that the vast majority of these patients seek treatment and are successfully started on cholesterol-lowering therapy to reduce their risk of premature cardiovascular disease .
	manualset3
124800	3	404442	13	NULL	NULL	0	NULL	FH patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings indicate not only that this case-finding approach is effective in identifying FH patients who otherwise would not have been identified but also that the vast majority of these patients seek treatment and are successfully started on cholesterol-lowering therapy to reduce their risk of premature cardiovascular disease .
	manualset3
124801	4	404442	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings indicate not only that this case-finding approach is effective in identifying FH patients who otherwise would not have been identified but also that the vast majority of these patients seek treatment and are successfully started on cholesterol-lowering therapy to reduce their risk of premature cardiovascular disease .
	manualset3
124802	5	404442	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings indicate not only that this case-finding approach is effective in identifying FH patients who otherwise would not have been identified but also that the vast majority of these patients seek treatment and are successfully started on cholesterol-lowering therapy to reduce their risk of premature cardiovascular disease .
	manualset3
124803	6	404442	13	NULL	NULL	0	NULL	cholesterol-lowering therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings indicate not only that this case-finding approach is effective in identifying FH patients who otherwise would not have been identified but also that the vast majority of these patients seek treatment and are successfully started on cholesterol-lowering therapy to reduce their risk of premature cardiovascular disease .
	manualset3
124804	7	404442	13	NULL	NULL	0	NULL	risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings indicate not only that this case-finding approach is effective in identifying FH patients who otherwise would not have been identified but also that the vast majority of these patients seek treatment and are successfully started on cholesterol-lowering therapy to reduce their risk of premature cardiovascular disease .
	manualset3
124806	8	404442	13	NULL	NULL	0	NULL	premature cardiovascular disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings indicate not only that this case-finding approach is effective in identifying FH patients who otherwise would not have been identified but also that the vast majority of these patients seek treatment and are successfully started on cholesterol-lowering therapy to reduce their risk of premature cardiovascular disease .
	manualset3
124808	1	404443	13	NULL	NULL	0	NULL	dose	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose of 2.5 mg/kg d , 1-propranolol , a beta adrenergic blocker , prevented the effect of 10 mg/kg salbutamol but the dose of 5 mg/kg did not significantly change the effect of 0.6 or 1.25 mg/kg d-amphetamine .
	manualset3
124810	2	404443	13	NULL	NULL	0	NULL	2.5 mg/kg d	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose of 2.5 mg/kg d , 1-propranolol , a beta adrenergic blocker , prevented the effect of 10 mg/kg salbutamol but the dose of 5 mg/kg did not significantly change the effect of 0.6 or 1.25 mg/kg d-amphetamine .
	manualset3
124811	3	404443	13	NULL	NULL	0	NULL	1-propranolol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose of 2.5 mg/kg d , 1-propranolol , a beta adrenergic blocker , prevented the effect of 10 mg/kg salbutamol but the dose of 5 mg/kg did not significantly change the effect of 0.6 or 1.25 mg/kg d-amphetamine .
	manualset3
124812	4	404443	13	NULL	NULL	0	NULL	beta adrenergic blocker	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose of 2.5 mg/kg d , 1-propranolol , a beta adrenergic blocker , prevented the effect of 10 mg/kg salbutamol but the dose of 5 mg/kg did not significantly change the effect of 0.6 or 1.25 mg/kg d-amphetamine .
	manualset3
124813	5	404443	13	NULL	NULL	0	NULL	effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose of 2.5 mg/kg d , 1-propranolol , a beta adrenergic blocker , prevented the effect of 10 mg/kg salbutamol but the dose of 5 mg/kg did not significantly change the effect of 0.6 or 1.25 mg/kg d-amphetamine .
	manualset3
124814	6	404443	13	NULL	NULL	0	NULL	10 mg/kg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose of 2.5 mg/kg d , 1-propranolol , a beta adrenergic blocker , prevented the effect of 10 mg/kg salbutamol but the dose of 5 mg/kg did not significantly change the effect of 0.6 or 1.25 mg/kg d-amphetamine .
	manualset3
124815	7	404443	13	NULL	NULL	0	NULL	salbutamol 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose of 2.5 mg/kg d , 1-propranolol , a beta adrenergic blocker , prevented the effect of 10 mg/kg salbutamol but the dose of 5 mg/kg did not significantly change the effect of 0.6 or 1.25 mg/kg d-amphetamine .
	manualset3
124816	8	404443	13	NULL	NULL	0	NULL	dose	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose of 2.5 mg/kg d , 1-propranolol , a beta adrenergic blocker , prevented the effect of 10 mg/kg salbutamol but the dose of 5 mg/kg did not significantly change the effect of 0.6 or 1.25 mg/kg d-amphetamine .
	manualset3
124818	9	404443	13	NULL	NULL	0	NULL	5 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose of 2.5 mg/kg d , 1-propranolol , a beta adrenergic blocker , prevented the effect of 10 mg/kg salbutamol but the dose of 5 mg/kg did not significantly change the effect of 0.6 or 1.25 mg/kg d-amphetamine .
	manualset3
124820	10	404443	13	NULL	NULL	0	NULL	effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose of 2.5 mg/kg d , 1-propranolol , a beta adrenergic blocker , prevented the effect of 10 mg/kg salbutamol but the dose of 5 mg/kg did not significantly change the effect of 0.6 or 1.25 mg/kg d-amphetamine .
	manualset3
124821	11	404443	13	NULL	NULL	NULL	NULL	0.6 mg/kg 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A dose of 2.5 mg/kg d , 1-propranolol , a beta adrenergic blocker , prevented the effect of 10 mg/kg salbutamol but the dose of 5 mg/kg did not significantly change the effect of 0.6 or 1.25 mg/kg d-amphetamine .
	manualset3
124822	12	404443	13	NULL	NULL	0	NULL	d-amphetamine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose of 2.5 mg/kg d , 1-propranolol , a beta adrenergic blocker , prevented the effect of 10 mg/kg salbutamol but the dose of 5 mg/kg did not significantly change the effect of 0.6 or 1.25 mg/kg d-amphetamine .
	manualset3
124825	13	404443	13	NULL	NULL	0	NULL	1.25 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A dose of 2.5 mg/kg d , 1-propranolol , a beta adrenergic blocker , prevented the effect of 10 mg/kg salbutamol but the dose of 5 mg/kg did not significantly change the effect of 0.6 or 1.25 mg/kg d-amphetamine .
	manualset3
124826	1	404444	13	NULL	NULL	0	NULL	findings	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings indicate that decitabine can relieve p21WAF1 repression in AML by a mechanism that involves release of HDAC1 without requiring promoter demethylation .
	manualset3
124827	2	404444	13	NULL	NULL	0	NULL	decitabine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings indicate that decitabine can relieve p21WAF1 repression in AML by a mechanism that involves release of HDAC1 without requiring promoter demethylation .
	manualset3
124828	3	404444	13	NULL	NULL	0	NULL	p21WAF1 repression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings indicate that decitabine can relieve p21WAF1 repression in AML by a mechanism that involves release of HDAC1 without requiring promoter demethylation .
	manualset3
124829	4	404444	13	NULL	NULL	0	NULL	AML	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings indicate that decitabine can relieve p21WAF1 repression in AML by a mechanism that involves release of HDAC1 without requiring promoter demethylation .
	manualset3
124830	5	404444	13	NULL	NULL	0	NULL	mechanism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings indicate that decitabine can relieve p21WAF1 repression in AML by a mechanism that involves release of HDAC1 without requiring promoter demethylation .
	manualset3
124831	6	404444	13	NULL	NULL	0	NULL	release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings indicate that decitabine can relieve p21WAF1 repression in AML by a mechanism that involves release of HDAC1 without requiring promoter demethylation .
	manualset3
124832	7	404444	13	NULL	NULL	0	NULL	HDAC1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings indicate that decitabine can relieve p21WAF1 repression in AML by a mechanism that involves release of HDAC1 without requiring promoter demethylation .
	manualset3
124833	8	404444	13	NULL	NULL	0	NULL	promoter demethylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings indicate that decitabine can relieve p21WAF1 repression in AML by a mechanism that involves release of HDAC1 without requiring promoter demethylation .
	manualset3
124834	1	404445	13	NULL	NULL	0	NULL	findings	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings provide evidence that curcuminoids target the FGF-2 angiogenic signaling pathway and inhibit expression of gelatinase B in the angiogenic process .
	manualset3
124835	2	404445	13	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings provide evidence that curcuminoids target the FGF-2 angiogenic signaling pathway and inhibit expression of gelatinase B in the angiogenic process .
	manualset3
124836	3	404445	13	NULL	NULL	0	NULL	curcuminoids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings provide evidence that curcuminoids target the FGF-2 angiogenic signaling pathway and inhibit expression of gelatinase B in the angiogenic process .
	manualset3
124838	5	404445	13	NULL	NULL	0	NULL	FGF-2 angiogenic signaling pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings provide evidence that curcuminoids target the FGF-2 angiogenic signaling pathway and inhibit expression of gelatinase B in the angiogenic process .
	manualset3
124839	6	404445	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings provide evidence that curcuminoids target the FGF-2 angiogenic signaling pathway and inhibit expression of gelatinase B in the angiogenic process .
	manualset3
124840	7	404445	13	NULL	NULL	0	NULL	gelatinase B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings provide evidence that curcuminoids target the FGF-2 angiogenic signaling pathway and inhibit expression of gelatinase B in the angiogenic process .
	manualset3
124841	8	404445	13	NULL	NULL	0	NULL	angiogenic process	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings provide evidence that curcuminoids target the FGF-2 angiogenic signaling pathway and inhibit expression of gelatinase B in the angiogenic process .
	manualset3
124842	1	404446	13	NULL	NULL	0	NULL	findings	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings provide the first direct evidence for the existence of a long-chain free fatty acid generation and export system in mitochondria and its activation in STZ-diabetic rat hearts in which FAO is enhanced .
	manualset3
124843	2	404446	13	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings provide the first direct evidence for the existence of a long-chain free fatty acid generation and export system in mitochondria and its activation in STZ-diabetic rat hearts in which FAO is enhanced .
	manualset3
124844	3	404446	13	NULL	NULL	0	NULL	existence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings provide the first direct evidence for the existence of a long-chain free fatty acid generation and export system in mitochondria and its activation in STZ-diabetic rat hearts in which FAO is enhanced .
	manualset3
124845	4	404446	13	NULL	NULL	0	NULL	long-chain free fatty acid generation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings provide the first direct evidence for the existence of a long-chain free fatty acid generation and export system in mitochondria and its activation in STZ-diabetic rat hearts in which FAO is enhanced .
	manualset3
124846	5	404446	13	NULL	NULL	0	NULL	export system 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings provide the first direct evidence for the existence of a long-chain free fatty acid generation and export system in mitochondria and its activation in STZ-diabetic rat hearts in which FAO is enhanced .
	manualset3
124847	6	404446	13	NULL	NULL	0	NULL	mitochondria	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings provide the first direct evidence for the existence of a long-chain free fatty acid generation and export system in mitochondria and its activation in STZ-diabetic rat hearts in which FAO is enhanced .
	manualset3
124848	7	404446	13	NULL	NULL	0	NULL	activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings provide the first direct evidence for the existence of a long-chain free fatty acid generation and export system in mitochondria and its activation in STZ-diabetic rat hearts in which FAO is enhanced .
	manualset3
124849	8	404446	13	NULL	NULL	0	NULL	STZ-diabetic rat hearts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings provide the first direct evidence for the existence of a long-chain free fatty acid generation and export system in mitochondria and its activation in STZ-diabetic rat hearts in which FAO is enhanced .
	manualset3
124850	9	404446	13	NULL	NULL	0	NULL	FAO 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings provide the first direct evidence for the existence of a long-chain free fatty acid generation and export system in mitochondria and its activation in STZ-diabetic rat hearts in which FAO is enhanced .
	manualset3
124851	1	404447	13	NULL	NULL	0	NULL	findings	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings reveal signals arising from differentiating cells that are required for maintaining progenitor cell quiescence and that function with the niche-derived signal in maintaining the progenitor state .
	manualset3
124852	2	404447	13	NULL	NULL	0	NULL	signals	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings reveal signals arising from differentiating cells that are required for maintaining progenitor cell quiescence and that function with the niche-derived signal in maintaining the progenitor state .
	manualset3
124853	3	404447	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings reveal signals arising from differentiating cells that are required for maintaining progenitor cell quiescence and that function with the niche-derived signal in maintaining the progenitor state .
	manualset3
124854	4	404447	13	NULL	NULL	0	NULL	progenitor cell quiescence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings reveal signals arising from differentiating cells that are required for maintaining progenitor cell quiescence and that function with the niche-derived signal in maintaining the progenitor state .
	manualset3
124855	5	404447	13	NULL	NULL	0	NULL	function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings reveal signals arising from differentiating cells that are required for maintaining progenitor cell quiescence and that function with the niche-derived signal in maintaining the progenitor state .
	manualset3
124856	6	404447	13	NULL	NULL	0	NULL	niche-derived signal 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings reveal signals arising from differentiating cells that are required for maintaining progenitor cell quiescence and that function with the niche-derived signal in maintaining the progenitor state .
	manualset3
124857	7	404447	13	NULL	NULL	0	NULL	progenitor state	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings reveal signals arising from differentiating cells that are required for maintaining progenitor cell quiescence and that function with the niche-derived signal in maintaining the progenitor state .
	manualset3
124983	1	404448	13	NULL	NULL	0	NULL	findings	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings reveal that for both the processes of acquisition and consolidation , treatment with nicotine ( 0.035 or 0.175 mg/kg , free base , sc ) shortened TL on the second day of the experiments ( TL2 ) , thus improving memory processes .
	manualset3
124984	2	404448	13	NULL	NULL	0	NULL	processes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings reveal that for both the processes of acquisition and consolidation , treatment with nicotine ( 0.035 or 0.175 mg/kg , free base , sc ) shortened TL on the second day of the experiments ( TL2 ) , thus improving memory processes .
	manualset3
124985	3	404448	13	NULL	NULL	0	NULL	acquisition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings reveal that for both the processes of acquisition and consolidation , treatment with nicotine ( 0.035 or 0.175 mg/kg , free base , sc ) shortened TL on the second day of the experiments ( TL2 ) , thus improving memory processes .
	manualset3
124986	4	404448	13	NULL	NULL	0	NULL	consolidation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings reveal that for both the processes of acquisition and consolidation , treatment with nicotine ( 0.035 or 0.175 mg/kg , free base , sc ) shortened TL on the second day of the experiments ( TL2 ) , thus improving memory processes .
	manualset3
124987	5	404448	13	NULL	NULL	0	NULL	treatment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings reveal that for both the processes of acquisition and consolidation , treatment with nicotine ( 0.035 or 0.175 mg/kg , free base , sc ) shortened TL on the second day of the experiments ( TL2 ) , thus improving memory processes .
	manualset3
124988	6	404448	13	NULL	NULL	0	NULL	nicotine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings reveal that for both the processes of acquisition and consolidation , treatment with nicotine ( 0.035 or 0.175 mg/kg , free base , sc ) shortened TL on the second day of the experiments ( TL2 ) , thus improving memory processes .
	manualset3
124989	7	404448	13	NULL	NULL	0	NULL	0.035 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings reveal that for both the processes of acquisition and consolidation , treatment with nicotine ( 0.035 or 0.175 mg/kg , free base , sc ) shortened TL on the second day of the experiments ( TL2 ) , thus improving memory processes .
	manualset3
124990	8	404448	13	NULL	NULL	0	NULL	0.175 mg/kg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings reveal that for both the processes of acquisition and consolidation , treatment with nicotine ( 0.035 or 0.175 mg/kg , free base , sc ) shortened TL on the second day of the experiments ( TL2 ) , thus improving memory processes .
	manualset3
124991	9	404448	13	NULL	NULL	0	NULL	TL	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings reveal that for both the processes of acquisition and consolidation , treatment with nicotine ( 0.035 or 0.175 mg/kg , free base , sc ) shortened TL on the second day of the experiments ( TL2 ) , thus improving memory processes .
	manualset3
124992	10	404448	13	NULL	NULL	0	NULL	second day	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings reveal that for both the processes of acquisition and consolidation , treatment with nicotine ( 0.035 or 0.175 mg/kg , free base , sc ) shortened TL on the second day of the experiments ( TL2 ) , thus improving memory processes .
	manualset3
124993	11	404448	13	NULL	NULL	0	NULL	experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings reveal that for both the processes of acquisition and consolidation , treatment with nicotine ( 0.035 or 0.175 mg/kg , free base , sc ) shortened TL on the second day of the experiments ( TL2 ) , thus improving memory processes .
	manualset3
124994	12	404448	13	NULL	NULL	0	NULL	TL2 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings reveal that for both the processes of acquisition and consolidation , treatment with nicotine ( 0.035 or 0.175 mg/kg , free base , sc ) shortened TL on the second day of the experiments ( TL2 ) , thus improving memory processes .
	manualset3
124995	13	404448	13	NULL	NULL	0	NULL	memory processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings reveal that for both the processes of acquisition and consolidation , treatment with nicotine ( 0.035 or 0.175 mg/kg , free base , sc ) shortened TL on the second day of the experiments ( TL2 ) , thus improving memory processes .
	manualset3
124996	1	404449	13	NULL	NULL	0	NULL	findings	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings reveal that male fertility is positively related to the proportion of male offspring .
	manualset3
124997	2	404449	13	NULL	NULL	0	NULL	male fertility 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings reveal that male fertility is positively related to the proportion of male offspring .
	manualset3
124998	3	404449	13	NULL	NULL	0	NULL	proportion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings reveal that male fertility is positively related to the proportion of male offspring .
	manualset3
124999	4	404449	13	NULL	NULL	0	NULL	male offspring 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings reveal that male fertility is positively related to the proportion of male offspring .
	manualset3
125000	1	404450	13	NULL	NULL	0	NULL	findings 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings show that the Syrian hamster is a promising immunocompetent model that is permissive to human adenovirus replication in tumors as well as normal tissues .
	manualset3
125001	2	404450	13	NULL	NULL	0	NULL	Syrian hamster	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings show that the Syrian hamster is a promising immunocompetent model that is permissive to human adenovirus replication in tumors as well as normal tissues .
	manualset3
125002	3	404450	13	NULL	NULL	0	NULL	immunocompetent model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings show that the Syrian hamster is a promising immunocompetent model that is permissive to human adenovirus replication in tumors as well as normal tissues .
	manualset3
125003	4	404450	13	NULL	NULL	0	NULL	human adenovirus replication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings show that the Syrian hamster is a promising immunocompetent model that is permissive to human adenovirus replication in tumors as well as normal tissues .
	manualset3
125004	5	404450	13	NULL	NULL	0	NULL	tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings show that the Syrian hamster is a promising immunocompetent model that is permissive to human adenovirus replication in tumors as well as normal tissues .
	manualset3
125005	6	404450	13	NULL	NULL	0	NULL	normal tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings show that the Syrian hamster is a promising immunocompetent model that is permissive to human adenovirus replication in tumors as well as normal tissues .
	manualset3
125006	1	404451	13	NULL	NULL	0	NULL	findings	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings showed that during the ` psychiatric care reform process , the nursing care provided by professionals kept presenting the segregating characteristics commonly-linked to the asylum care model , and that changes happened due to the influence of new routines and training these professionals were exposed to .
	manualset3
125007	2	404451	13	NULL	NULL	0	NULL	psychiatric care 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings showed that during the ` psychiatric care reform process , the nursing care provided by professionals kept presenting the segregating characteristics commonly-linked to the asylum care model , and that changes happened due to the influence of new routines and training these professionals were exposed to .
	manualset3
125008	3	404451	13	NULL	NULL	0	NULL	reform process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings showed that during the ` psychiatric care reform process , the nursing care provided by professionals kept presenting the segregating characteristics commonly-linked to the asylum care model , and that changes happened due to the influence of new routines and training these professionals were exposed to .
	manualset3
125009	4	404451	13	NULL	NULL	0	NULL	nursing care 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings showed that during the ` psychiatric care reform process , the nursing care provided by professionals kept presenting the segregating characteristics commonly-linked to the asylum care model , and that changes happened due to the influence of new routines and training these professionals were exposed to .
	manualset3
125010	5	404451	13	NULL	NULL	0	NULL	professionals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings showed that during the ` psychiatric care reform process , the nursing care provided by professionals kept presenting the segregating characteristics commonly-linked to the asylum care model , and that changes happened due to the influence of new routines and training these professionals were exposed to .
	manualset3
125011	6	404451	13	NULL	NULL	0	NULL	characteristics 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings showed that during the ` psychiatric care reform process , the nursing care provided by professionals kept presenting the segregating characteristics commonly-linked to the asylum care model , and that changes happened due to the influence of new routines and training these professionals were exposed to .
	manualset3
125012	7	404451	13	NULL	NULL	0	NULL	asylum care model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings showed that during the ` psychiatric care reform process , the nursing care provided by professionals kept presenting the segregating characteristics commonly-linked to the asylum care model , and that changes happened due to the influence of new routines and training these professionals were exposed to .
	manualset3
125013	8	404451	13	NULL	NULL	0	NULL	influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings showed that during the ` psychiatric care reform process , the nursing care provided by professionals kept presenting the segregating characteristics commonly-linked to the asylum care model , and that changes happened due to the influence of new routines and training these professionals were exposed to .
	manualset3
125014	9	404451	13	NULL	NULL	0	NULL	routines	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings showed that during the ` psychiatric care reform process , the nursing care provided by professionals kept presenting the segregating characteristics commonly-linked to the asylum care model , and that changes happened due to the influence of new routines and training these professionals were exposed to .
	manualset3
125015	10	404451	13	NULL	NULL	0	NULL	professionals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings showed that during the ` psychiatric care reform process , the nursing care provided by professionals kept presenting the segregating characteristics commonly-linked to the asylum care model , and that changes happened due to the influence of new routines and training these professionals were exposed to .
	manualset3
128810	11	404451	13	NULL	NULL	0	NULL	training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings showed that during the ` psychiatric care reform process , the nursing care provided by professionals kept presenting the segregating characteristics commonly-linked to the asylum care model , and that changes happened due to the influence of new routines and training these professionals were exposed to .
	manualset3
125016	1	404452	13	NULL	NULL	0	NULL	findings	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest an increase in Tc2 cell number in blood from psoriatic patients , and the association of Tc2 cells with inflammation in psoriasis .
	manualset3
125017	2	404452	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest an increase in Tc2 cell number in blood from psoriatic patients , and the association of Tc2 cells with inflammation in psoriasis .
	manualset3
125018	3	404452	13	NULL	NULL	0	NULL	Tc2 cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest an increase in Tc2 cell number in blood from psoriatic patients , and the association of Tc2 cells with inflammation in psoriasis .
	manualset3
125019	4	404452	13	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest an increase in Tc2 cell number in blood from psoriatic patients , and the association of Tc2 cells with inflammation in psoriasis .
	manualset3
125020	5	404452	13	NULL	NULL	0	NULL	blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest an increase in Tc2 cell number in blood from psoriatic patients , and the association of Tc2 cells with inflammation in psoriasis .
	manualset3
125021	6	404452	13	NULL	NULL	0	NULL	psoriatic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest an increase in Tc2 cell number in blood from psoriatic patients , and the association of Tc2 cells with inflammation in psoriasis .
	manualset3
125022	7	404452	13	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest an increase in Tc2 cell number in blood from psoriatic patients , and the association of Tc2 cells with inflammation in psoriasis .
	manualset3
125023	8	404452	13	NULL	NULL	0	NULL	Tc2 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest an increase in Tc2 cell number in blood from psoriatic patients , and the association of Tc2 cells with inflammation in psoriasis .
	manualset3
125024	9	404452	13	NULL	NULL	0	NULL	inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest an increase in Tc2 cell number in blood from psoriatic patients , and the association of Tc2 cells with inflammation in psoriasis .
	manualset3
125025	10	404452	13	NULL	NULL	0	NULL	psoriasis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest an increase in Tc2 cell number in blood from psoriatic patients , and the association of Tc2 cells with inflammation in psoriasis .
	manualset3
125026	1	404453	13	NULL	NULL	0	NULL	double-blind controlled trial 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A double-blind controlled trial of long-acting quinidine bisulphate .
	manualset3
125027	2	404453	13	NULL	NULL	0	NULL	quinidine bisulphate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A double-blind controlled trial of long-acting quinidine bisulphate .
	manualset3
125028	1	404454	13	NULL	NULL	0	NULL	findings	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that JKD directly regulates SCR and MGP expression in cooperation with SHR , SCR and MGP .
	manualset3
125029	2	404454	13	NULL	NULL	0	NULL	JKD 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that JKD directly regulates SCR and MGP expression in cooperation with SHR , SCR and MGP .
	manualset3
125030	3	404454	13	NULL	NULL	0	NULL	SCR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that JKD directly regulates SCR and MGP expression in cooperation with SHR , SCR and MGP .
	manualset3
125031	4	404454	13	NULL	NULL	0	NULL	MGP 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that JKD directly regulates SCR and MGP expression in cooperation with SHR , SCR and MGP .
	manualset3
125032	5	404454	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that JKD directly regulates SCR and MGP expression in cooperation with SHR , SCR and MGP .
	manualset3
125033	6	404454	13	NULL	NULL	0	NULL	cooperation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that JKD directly regulates SCR and MGP expression in cooperation with SHR , SCR and MGP .
	manualset3
125034	7	404454	13	NULL	NULL	0	NULL	SHR 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that JKD directly regulates SCR and MGP expression in cooperation with SHR , SCR and MGP .
	manualset3
125035	8	404454	13	NULL	NULL	0	NULL	SCR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that JKD directly regulates SCR and MGP expression in cooperation with SHR , SCR and MGP .
	manualset3
125036	9	404454	13	NULL	NULL	0	NULL	MGP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that JKD directly regulates SCR and MGP expression in cooperation with SHR , SCR and MGP .
	manualset3
125037	1	404455	13	NULL	NULL	0	NULL	findings 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that for runs of or around ten generations ' duration-as is typical in DE-there is little difference between the way in which DE needs to be configured in the high - and low-throughput regimes , nor across different degrees of landscape epistasis .
	manualset3
125038	2	404455	13	NULL	NULL	0	NULL	runs	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that for runs of or around ten generations ' duration-as is typical in DE-there is little difference between the way in which DE needs to be configured in the high - and low-throughput regimes , nor across different degrees of landscape epistasis .
	manualset3
125039	3	404455	13	NULL	NULL	0	NULL	ten generations 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that for runs of or around ten generations ' duration-as is typical in DE-there is little difference between the way in which DE needs to be configured in the high - and low-throughput regimes , nor across different degrees of landscape epistasis .
	manualset3
125040	4	404455	13	NULL	NULL	0	NULL	duration-as	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that for runs of or around ten generations ' duration-as is typical in DE-there is little difference between the way in which DE needs to be configured in the high - and low-throughput regimes , nor across different degrees of landscape epistasis .
	manualset3
125041	5	404455	13	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that for runs of or around ten generations ' duration-as is typical in DE-there is little difference between the way in which DE needs to be configured in the high - and low-throughput regimes , nor across different degrees of landscape epistasis .
	manualset3
125042	6	404455	13	NULL	NULL	0	NULL	way	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that for runs of or around ten generations ' duration-as is typical in DE-there is little difference between the way in which DE needs to be configured in the high - and low-throughput regimes , nor across different degrees of landscape epistasis .
	manualset3
125043	7	404455	13	NULL	NULL	0	NULL	DE	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that for runs of or around ten generations ' duration-as is typical in DE-there is little difference between the way in which DE needs to be configured in the high - and low-throughput regimes , nor across different degrees of landscape epistasis .
	manualset3
125044	8	404455	13	NULL	NULL	0	NULL	high -throughput regimes	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that for runs of or around ten generations ' duration-as is typical in DE-there is little difference between the way in which DE needs to be configured in the high - and low-throughput regimes , nor across different degrees of landscape epistasis .
	manualset3
125045	9	404455	13	NULL	NULL	0	NULL	low-throughput regimes	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that for runs of or around ten generations ' duration-as is typical in DE-there is little difference between the way in which DE needs to be configured in the high - and low-throughput regimes , nor across different degrees of landscape epistasis .
	manualset3
125046	10	404455	13	NULL	NULL	0	NULL	degrees 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that for runs of or around ten generations ' duration-as is typical in DE-there is little difference between the way in which DE needs to be configured in the high - and low-throughput regimes , nor across different degrees of landscape epistasis .
	manualset3
125047	11	404455	13	NULL	NULL	0	NULL	landscape epistasis	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that for runs of or around ten generations ' duration-as is typical in DE-there is little difference between the way in which DE needs to be configured in the high - and low-throughput regimes , nor across different degrees of landscape epistasis .
	manualset3
125048	1	404456	13	NULL	NULL	0	NULL	findings	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that improved maternal health education and care in all communities may reduce the burden of fetal loss in this province .
	manualset3
125049	2	404456	13	NULL	NULL	0	NULL	maternal health education	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that improved maternal health education and care in all communities may reduce the burden of fetal loss in this province .
	manualset3
125050	3	404456	13	NULL	NULL	0	NULL	maternal health care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that improved maternal health education and care in all communities may reduce the burden of fetal loss in this province .
	manualset3
125051	4	404456	13	NULL	NULL	0	NULL	communities	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that improved maternal health education and care in all communities may reduce the burden of fetal loss in this province .
	manualset3
125052	5	404456	13	NULL	NULL	0	NULL	burden	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that improved maternal health education and care in all communities may reduce the burden of fetal loss in this province .
	manualset3
125053	6	404456	13	NULL	NULL	0	NULL	fetal loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that improved maternal health education and care in all communities may reduce the burden of fetal loss in this province .
	manualset3
125054	7	404456	13	NULL	NULL	0	NULL	province	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that improved maternal health education and care in all communities may reduce the burden of fetal loss in this province .
	manualset3
125055	1	404457	13	NULL	NULL	0	NULL	findings	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that neutrophil defensins have the potential to modulate the inflammatory responses through regulation of cytokine production and adhesion molecule expression .
	manualset3
125056	2	404457	13	NULL	NULL	0	NULL	neutrophil defensins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that neutrophil defensins have the potential to modulate the inflammatory responses through regulation of cytokine production and adhesion molecule expression .
	manualset3
125057	3	404457	13	NULL	NULL	0	NULL	 inflammatory responses 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that neutrophil defensins have the potential to modulate the inflammatory responses through regulation of cytokine production and adhesion molecule expression .
	manualset3
125058	4	404457	13	NULL	NULL	0	NULL	regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that neutrophil defensins have the potential to modulate the inflammatory responses through regulation of cytokine production and adhesion molecule expression .
	manualset3
125059	5	404457	13	NULL	NULL	0	NULL	cytokine production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that neutrophil defensins have the potential to modulate the inflammatory responses through regulation of cytokine production and adhesion molecule expression .
	manualset3
125060	6	404457	13	NULL	NULL	0	NULL	adhesion molecule expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that neutrophil defensins have the potential to modulate the inflammatory responses through regulation of cytokine production and adhesion molecule expression .
	manualset3
125061	1	404458	13	NULL	NULL	0	NULL	findings	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that the Hebb repetition effect can be associated with response learning as well as stimulus processing .
	manualset3
125062	2	404458	13	NULL	NULL	0	NULL	Hebb repetition effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that the Hebb repetition effect can be associated with response learning as well as stimulus processing .
	manualset3
125063	3	404458	13	NULL	NULL	0	NULL	response learning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that the Hebb repetition effect can be associated with response learning as well as stimulus processing .
	manualset3
125064	4	404458	13	NULL	NULL	0	NULL	stimulus processing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings suggest that the Hebb repetition effect can be associated with response learning as well as stimulus processing .
	manualset3
125065	1	404459	13	NULL	NULL	0	NULL	findings	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings support that G-protein coupling and preference is dominated by specific structural features at the intracellular region of the activated GPCR but is completed by additional complementary recognition patterns between receptor and G-protein subtypes .
	manualset3
125066	2	404459	13	NULL	NULL	0	NULL	G-protein coupling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings support that G-protein coupling and preference is dominated by specific structural features at the intracellular region of the activated GPCR but is completed by additional complementary recognition patterns between receptor and G-protein subtypes .
	manualset3
125067	3	404459	13	NULL	NULL	0	NULL	preference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings support that G-protein coupling and preference is dominated by specific structural features at the intracellular region of the activated GPCR but is completed by additional complementary recognition patterns between receptor and G-protein subtypes .
	manualset3
125068	4	404459	13	NULL	NULL	0	NULL	structural features	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings support that G-protein coupling and preference is dominated by specific structural features at the intracellular region of the activated GPCR but is completed by additional complementary recognition patterns between receptor and G-protein subtypes .
	manualset3
125069	5	404459	13	NULL	NULL	0	NULL	intracellular region	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings support that G-protein coupling and preference is dominated by specific structural features at the intracellular region of the activated GPCR but is completed by additional complementary recognition patterns between receptor and G-protein subtypes .
	manualset3
125070	6	404459	13	NULL	NULL	0	NULL	GPCR 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings support that G-protein coupling and preference is dominated by specific structural features at the intracellular region of the activated GPCR but is completed by additional complementary recognition patterns between receptor and G-protein subtypes .
	manualset3
125071	7	404459	13	NULL	NULL	0	NULL	complementary recognition patterns	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings support that G-protein coupling and preference is dominated by specific structural features at the intracellular region of the activated GPCR but is completed by additional complementary recognition patterns between receptor and G-protein subtypes .
	manualset3
125072	8	404459	13	NULL	NULL	0	NULL	receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings support that G-protein coupling and preference is dominated by specific structural features at the intracellular region of the activated GPCR but is completed by additional complementary recognition patterns between receptor and G-protein subtypes .
	manualset3
125073	9	404459	13	NULL	NULL	0	NULL	G-protein subtypes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings support that G-protein coupling and preference is dominated by specific structural features at the intracellular region of the activated GPCR but is completed by additional complementary recognition patterns between receptor and G-protein subtypes .
	manualset3
125074	1	404460	13	NULL	NULL	0	NULL	findings 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings unveil a differential role of derepressed Ink4a and Arf on HSCs and their BM microenvironment in Bmi1-deficient mice .
	manualset3
125075	2	404460	13	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings unveil a differential role of derepressed Ink4a and Arf on HSCs and their BM microenvironment in Bmi1-deficient mice .
	manualset3
125076	3	404460	13	NULL	NULL	0	NULL	Ink4a 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings unveil a differential role of derepressed Ink4a and Arf on HSCs and their BM microenvironment in Bmi1-deficient mice .
	manualset3
125077	4	404460	13	NULL	NULL	0	NULL	Arf 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings unveil a differential role of derepressed Ink4a and Arf on HSCs and their BM microenvironment in Bmi1-deficient mice .
	manualset3
125078	5	404460	13	NULL	NULL	0	NULL	HSCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings unveil a differential role of derepressed Ink4a and Arf on HSCs and their BM microenvironment in Bmi1-deficient mice .
	manualset3
125079	6	404460	13	NULL	NULL	0	NULL	BM microenvironment	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings unveil a differential role of derepressed Ink4a and Arf on HSCs and their BM microenvironment in Bmi1-deficient mice .
	manualset3
125080	7	404460	13	NULL	NULL	0	NULL	Bmi1-deficient mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings unveil a differential role of derepressed Ink4a and Arf on HSCs and their BM microenvironment in Bmi1-deficient mice .
	manualset3
125081	1	404461	13	NULL	NULL	0	NULL	laboratory	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Our laboratory revealed the close relationship between the vascular RAS and the action of insulin on the vasculature .
	manualset3
125082	2	404461	13	NULL	NULL	0	NULL	relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Our laboratory revealed the close relationship between the vascular RAS and the action of insulin on the vasculature .
	manualset3
125083	3	404461	13	NULL	NULL	0	NULL	RAS 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our laboratory revealed the close relationship between the vascular RAS and the action of insulin on the vasculature .
	manualset3
125084	4	404461	13	NULL	NULL	0	NULL	action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our laboratory revealed the close relationship between the vascular RAS and the action of insulin on the vasculature .
	manualset3
125085	5	404461	13	NULL	NULL	0	NULL	insulin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our laboratory revealed the close relationship between the vascular RAS and the action of insulin on the vasculature .
	manualset3
125086	6	404461	13	NULL	NULL	0	NULL	vasculature	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our laboratory revealed the close relationship between the vascular RAS and the action of insulin on the vasculature .
	manualset3
125087	1	404462	13	NULL	NULL	0	NULL	method 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Our method could be usefully exploited for comparative studies of rabbit and human PMNs with a cellular model of inflammatory oxidative stress in which the monitoring parameters are ROS and elastase .
	manualset3
125088	2	404462	13	NULL	NULL	0	NULL	comparative studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our method could be usefully exploited for comparative studies of rabbit and human PMNs with a cellular model of inflammatory oxidative stress in which the monitoring parameters are ROS and elastase .
	manualset3
125089	3	404462	13	NULL	NULL	0	NULL	rabbit PMNs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our method could be usefully exploited for comparative studies of rabbit and human PMNs with a cellular model of inflammatory oxidative stress in which the monitoring parameters are ROS and elastase .
	manualset3
125090	4	404462	13	NULL	NULL	0	NULL	human PMNs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our method could be usefully exploited for comparative studies of rabbit and human PMNs with a cellular model of inflammatory oxidative stress in which the monitoring parameters are ROS and elastase .
	manualset3
125091	5	404462	13	NULL	NULL	0	NULL	cellular model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Our method could be usefully exploited for comparative studies of rabbit and human PMNs with a cellular model of inflammatory oxidative stress in which the monitoring parameters are ROS and elastase .
	manualset3
125092	6	404462	13	NULL	NULL	0	NULL	inflammatory oxidative stress 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our method could be usefully exploited for comparative studies of rabbit and human PMNs with a cellular model of inflammatory oxidative stress in which the monitoring parameters are ROS and elastase .
	manualset3
125093	7	404462	13	NULL	NULL	0	NULL	monitoring parameters	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our method could be usefully exploited for comparative studies of rabbit and human PMNs with a cellular model of inflammatory oxidative stress in which the monitoring parameters are ROS and elastase .
	manualset3
125094	8	404462	13	NULL	NULL	0	NULL	ROS 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our method could be usefully exploited for comparative studies of rabbit and human PMNs with a cellular model of inflammatory oxidative stress in which the monitoring parameters are ROS and elastase .
	manualset3
125095	9	404462	13	NULL	NULL	0	NULL	elastase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our method could be usefully exploited for comparative studies of rabbit and human PMNs with a cellular model of inflammatory oxidative stress in which the monitoring parameters are ROS and elastase .
	manualset3
125096	1	404463	13	NULL	NULL	0	NULL	method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Our method may prove useful as a new form of cancer gene therapy in the future .
	manualset3
125097	2	404463	13	NULL	NULL	0	NULL	new form	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our method may prove useful as a new form of cancer gene therapy in the future .
	manualset3
125098	3	404463	13	NULL	NULL	0	NULL	cancer gene therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our method may prove useful as a new form of cancer gene therapy in the future .
	manualset3
125099	4	404463	13	NULL	NULL	0	NULL	future	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Our method may prove useful as a new form of cancer gene therapy in the future .
	manualset3
125100	1	404464	13	NULL	NULL	0	NULL	objective	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to determine if the All-Patient Refined Diagnosis-Related Groups ( APR-DRGs ) and other comorbidity scores correlate with pain level , functional abilities , and hospital cost after primary total joint arthroplasty ( TJA ) .
	manualset3
125101	2	404464	13	NULL	NULL	0	NULL	All-Patient Refined Diagnosis-Related Groups ( APR-DRGs )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to determine if the All-Patient Refined Diagnosis-Related Groups ( APR-DRGs ) and other comorbidity scores correlate with pain level , functional abilities , and hospital cost after primary total joint arthroplasty ( TJA ) .
	manualset3
125102	3	404464	13	NULL	NULL	0	NULL	comorbidity scores	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to determine if the All-Patient Refined Diagnosis-Related Groups ( APR-DRGs ) and other comorbidity scores correlate with pain level , functional abilities , and hospital cost after primary total joint arthroplasty ( TJA ) .
	manualset3
125103	4	404464	13	NULL	NULL	0	NULL	pain level	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to determine if the All-Patient Refined Diagnosis-Related Groups ( APR-DRGs ) and other comorbidity scores correlate with pain level , functional abilities , and hospital cost after primary total joint arthroplasty ( TJA ) .
	manualset3
125104	5	404464	13	NULL	NULL	0	NULL	functional abilities 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to determine if the All-Patient Refined Diagnosis-Related Groups ( APR-DRGs ) and other comorbidity scores correlate with pain level , functional abilities , and hospital cost after primary total joint arthroplasty ( TJA ) .
	manualset3
125105	6	404464	13	NULL	NULL	0	NULL	hospital cost	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to determine if the All-Patient Refined Diagnosis-Related Groups ( APR-DRGs ) and other comorbidity scores correlate with pain level , functional abilities , and hospital cost after primary total joint arthroplasty ( TJA ) .
	manualset3
125106	7	404464	13	NULL	NULL	0	NULL	primary total joint arthroplasty ( TJA )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to determine if the All-Patient Refined Diagnosis-Related Groups ( APR-DRGs ) and other comorbidity scores correlate with pain level , functional abilities , and hospital cost after primary total joint arthroplasty ( TJA ) .
	manualset3
125107	1	404465	13	NULL	NULL	0	NULL	objective	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to investigate the relationships between organochlorine concentrations in different biological media .
	manualset3
125108	2	404465	13	NULL	NULL	0	NULL	relationships 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to investigate the relationships between organochlorine concentrations in different biological media .
	manualset3
125109	3	404465	13	NULL	NULL	0	NULL	organochlorine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to investigate the relationships between organochlorine concentrations in different biological media .
	manualset3
125110	4	404465	13	NULL	NULL	0	NULL	concentrations 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to investigate the relationships between organochlorine concentrations in different biological media .
	manualset3
125111	5	404465	13	NULL	NULL	0	NULL	biological media 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to investigate the relationships between organochlorine concentrations in different biological media .
	manualset3
125112	1	404466	13	NULL	NULL	0	NULL	objective	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to investigate whether PLA2 is present in meconium and inhibits pulmonary surfactant activity in vitro .
	manualset3
125113	2	404466	13	NULL	NULL	0	NULL	PLA2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to investigate whether PLA2 is present in meconium and inhibits pulmonary surfactant activity in vitro .
	manualset3
125114	3	404466	13	NULL	NULL	0	NULL	meconium 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to investigate whether PLA2 is present in meconium and inhibits pulmonary surfactant activity in vitro .
	manualset3
125115	4	404466	13	NULL	NULL	0	NULL	pulmonary surfactant activity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to investigate whether PLA2 is present in meconium and inhibits pulmonary surfactant activity in vitro .
	manualset3
125116	1	404467	13	NULL	NULL	0	NULL	objective 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to test the hypothesis that people with PsA have poorer QoL than patients with PsC because of the added burden of arthritis , age and comorbidities .
	manualset3
125117	2	404467	13	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to test the hypothesis that people with PsA have poorer QoL than patients with PsC because of the added burden of arthritis , age and comorbidities .
	manualset3
125118	3	404467	13	NULL	NULL	0	NULL	people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to test the hypothesis that people with PsA have poorer QoL than patients with PsC because of the added burden of arthritis , age and comorbidities .
	manualset3
125119	4	404467	13	NULL	NULL	0	NULL	PsA	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to test the hypothesis that people with PsA have poorer QoL than patients with PsC because of the added burden of arthritis , age and comorbidities .
	manualset3
125120	5	404467	13	NULL	NULL	0	NULL	QoL	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to test the hypothesis that people with PsA have poorer QoL than patients with PsC because of the added burden of arthritis , age and comorbidities .
	manualset3
125121	6	404467	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to test the hypothesis that people with PsA have poorer QoL than patients with PsC because of the added burden of arthritis , age and comorbidities .
	manualset3
125122	7	404467	13	NULL	NULL	0	NULL	PsC 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to test the hypothesis that people with PsA have poorer QoL than patients with PsC because of the added burden of arthritis , age and comorbidities .
	manualset3
125123	8	404467	13	NULL	NULL	0	NULL	burden of arthritis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to test the hypothesis that people with PsA have poorer QoL than patients with PsC because of the added burden of arthritis , age and comorbidities .
	manualset3
125124	9	404467	13	NULL	NULL	0	NULL	age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to test the hypothesis that people with PsA have poorer QoL than patients with PsC because of the added burden of arthritis , age and comorbidities .
	manualset3
125125	10	404467	13	NULL	NULL	0	NULL	comorbidities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to test the hypothesis that people with PsA have poorer QoL than patients with PsC because of the added burden of arthritis , age and comorbidities .
	manualset3
125126	1	404468	13	NULL	NULL	0	NULL	objective	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to use a calibrated and validated simulation of HIV disease to estimate the impact of alcohol on survival .
	manualset3
125127	2	404468	13	NULL	NULL	0	NULL	simulation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to use a calibrated and validated simulation of HIV disease to estimate the impact of alcohol on survival .
	manualset3
125128	3	404468	13	NULL	NULL	0	NULL	HIV disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to use a calibrated and validated simulation of HIV disease to estimate the impact of alcohol on survival .
	manualset3
125129	4	404468	13	NULL	NULL	0	NULL	impact 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to use a calibrated and validated simulation of HIV disease to estimate the impact of alcohol on survival .
	manualset3
125130	5	404468	13	NULL	NULL	0	NULL	alcohol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to use a calibrated and validated simulation of HIV disease to estimate the impact of alcohol on survival .
	manualset3
125131	6	404468	13	NULL	NULL	0	NULL	survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to use a calibrated and validated simulation of HIV disease to estimate the impact of alcohol on survival .
	manualset3
125132	1	404469	13	NULL	NULL	0	NULL	objective	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to use electrophysiology to test the hypothesis of gradual and sequential involvement of the amygdala and then cortex during audiogenic kindling .
	manualset3
125133	2	404469	13	NULL	NULL	0	NULL	electrophysiology 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to use electrophysiology to test the hypothesis of gradual and sequential involvement of the amygdala and then cortex during audiogenic kindling .
	manualset3
125134	3	404469	13	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to use electrophysiology to test the hypothesis of gradual and sequential involvement of the amygdala and then cortex during audiogenic kindling .
	manualset3
125135	4	404469	13	NULL	NULL	0	NULL	gradual involvement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to use electrophysiology to test the hypothesis of gradual and sequential involvement of the amygdala and then cortex during audiogenic kindling .
	manualset3
125136	5	404469	13	NULL	NULL	0	NULL	sequential involvement 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to use electrophysiology to test the hypothesis of gradual and sequential involvement of the amygdala and then cortex during audiogenic kindling .
	manualset3
125137	6	404469	13	NULL	NULL	0	NULL	amygdala	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to use electrophysiology to test the hypothesis of gradual and sequential involvement of the amygdala and then cortex during audiogenic kindling .
	manualset3
125138	7	404469	13	NULL	NULL	0	NULL	cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to use electrophysiology to test the hypothesis of gradual and sequential involvement of the amygdala and then cortex during audiogenic kindling .
	manualset3
125139	8	404469	13	NULL	NULL	0	NULL	audiogenic kindling	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objective was to use electrophysiology to test the hypothesis of gradual and sequential involvement of the amygdala and then cortex during audiogenic kindling .
	manualset3
125140	1	404470	13	NULL	NULL	0	NULL	objectives	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objectives were to compare the EMG and force generated by the ankle plantar - and dorsi-flexors in normal and spastic hemiparetic subjects , and to investigate their reproducibility and their correlation with clinical spasticity .
	manualset3
125141	2	404470	13	NULL	NULL	0	NULL	EMG	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objectives were to compare the EMG and force generated by the ankle plantar - and dorsi-flexors in normal and spastic hemiparetic subjects , and to investigate their reproducibility and their correlation with clinical spasticity .
	manualset3
125142	3	404470	13	NULL	NULL	0	NULL	force 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objectives were to compare the EMG and force generated by the ankle plantar - and dorsi-flexors in normal and spastic hemiparetic subjects , and to investigate their reproducibility and their correlation with clinical spasticity .
	manualset3
125143	4	404470	13	NULL	NULL	0	NULL	ankle plantar	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objectives were to compare the EMG and force generated by the ankle plantar - and dorsi-flexors in normal and spastic hemiparetic subjects , and to investigate their reproducibility and their correlation with clinical spasticity .
	manualset3
125144	5	404470	13	NULL	NULL	0	NULL	dorsi-flexors	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objectives were to compare the EMG and force generated by the ankle plantar - and dorsi-flexors in normal and spastic hemiparetic subjects , and to investigate their reproducibility and their correlation with clinical spasticity .
	manualset3
125145	6	404470	13	NULL	NULL	0	NULL	normal subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objectives were to compare the EMG and force generated by the ankle plantar - and dorsi-flexors in normal and spastic hemiparetic subjects , and to investigate their reproducibility and their correlation with clinical spasticity .
	manualset3
125146	7	404470	13	NULL	NULL	0	NULL	spastic hemiparetic subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objectives were to compare the EMG and force generated by the ankle plantar - and dorsi-flexors in normal and spastic hemiparetic subjects , and to investigate their reproducibility and their correlation with clinical spasticity .
	manualset3
125147	8	404470	13	NULL	NULL	0	NULL	reproducibility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objectives were to compare the EMG and force generated by the ankle plantar - and dorsi-flexors in normal and spastic hemiparetic subjects , and to investigate their reproducibility and their correlation with clinical spasticity .
	manualset3
125148	9	404470	13	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objectives were to compare the EMG and force generated by the ankle plantar - and dorsi-flexors in normal and spastic hemiparetic subjects , and to investigate their reproducibility and their correlation with clinical spasticity .
	manualset3
125149	10	404470	13	NULL	NULL	0	NULL	clinical spasticity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our objectives were to compare the EMG and force generated by the ankle plantar - and dorsi-flexors in normal and spastic hemiparetic subjects , and to investigate their reproducibility and their correlation with clinical spasticity .
	manualset3
125150	1	404471	13	NULL	NULL	0	NULL	double-blind study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A double-blind study was performed on 10 patients with type 1 diabetes mellitus ( DM ) without CF ( 3 male , 7 female , mean age 25.5 years ) and 9 patients with insulin-dependent CF-related diabetes ( CFRD ) ( 8 male , 1 female , mean age 21.9 years ) .
	manualset3
125151	2	404471	13	NULL	NULL	0	NULL	10 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A double-blind study was performed on 10 patients with type 1 diabetes mellitus ( DM ) without CF ( 3 male , 7 female , mean age 25.5 years ) and 9 patients with insulin-dependent CF-related diabetes ( CFRD ) ( 8 male , 1 female , mean age 21.9 years ) .
	manualset3
125152	3	404471	13	NULL	NULL	0	NULL	type 1 diabetes mellitus ( DM )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A double-blind study was performed on 10 patients with type 1 diabetes mellitus ( DM ) without CF ( 3 male , 7 female , mean age 25.5 years ) and 9 patients with insulin-dependent CF-related diabetes ( CFRD ) ( 8 male , 1 female , mean age 21.9 years ) .
	manualset3
125153	4	404471	13	NULL	NULL	0	NULL	CF	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A double-blind study was performed on 10 patients with type 1 diabetes mellitus ( DM ) without CF ( 3 male , 7 female , mean age 25.5 years ) and 9 patients with insulin-dependent CF-related diabetes ( CFRD ) ( 8 male , 1 female , mean age 21.9 years ) .
	manualset3
125154	5	404471	13	NULL	NULL	0	NULL	3 male	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A double-blind study was performed on 10 patients with type 1 diabetes mellitus ( DM ) without CF ( 3 male , 7 female , mean age 25.5 years ) and 9 patients with insulin-dependent CF-related diabetes ( CFRD ) ( 8 male , 1 female , mean age 21.9 years ) .
	manualset3
125155	6	404471	13	NULL	NULL	0	NULL	7 female	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A double-blind study was performed on 10 patients with type 1 diabetes mellitus ( DM ) without CF ( 3 male , 7 female , mean age 25.5 years ) and 9 patients with insulin-dependent CF-related diabetes ( CFRD ) ( 8 male , 1 female , mean age 21.9 years ) .
	manualset3
125156	7	404471	13	NULL	NULL	0	NULL	mean age 25.5 years	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A double-blind study was performed on 10 patients with type 1 diabetes mellitus ( DM ) without CF ( 3 male , 7 female , mean age 25.5 years ) and 9 patients with insulin-dependent CF-related diabetes ( CFRD ) ( 8 male , 1 female , mean age 21.9 years ) .
	manualset3
125157	8	404471	13	NULL	NULL	0	NULL	9 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A double-blind study was performed on 10 patients with type 1 diabetes mellitus ( DM ) without CF ( 3 male , 7 female , mean age 25.5 years ) and 9 patients with insulin-dependent CF-related diabetes ( CFRD ) ( 8 male , 1 female , mean age 21.9 years ) .
	manualset3
125158	9	404471	13	NULL	NULL	0	NULL	insulin-dependent CF-related diabetes ( CFRD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A double-blind study was performed on 10 patients with type 1 diabetes mellitus ( DM ) without CF ( 3 male , 7 female , mean age 25.5 years ) and 9 patients with insulin-dependent CF-related diabetes ( CFRD ) ( 8 male , 1 female , mean age 21.9 years ) .
	manualset3
125159	10	404471	13	NULL	NULL	0	NULL	8 male	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A double-blind study was performed on 10 patients with type 1 diabetes mellitus ( DM ) without CF ( 3 male , 7 female , mean age 25.5 years ) and 9 patients with insulin-dependent CF-related diabetes ( CFRD ) ( 8 male , 1 female , mean age 21.9 years ) .
	manualset3
125160	11	404471	13	NULL	NULL	0	NULL	1 female	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A double-blind study was performed on 10 patients with type 1 diabetes mellitus ( DM ) without CF ( 3 male , 7 female , mean age 25.5 years ) and 9 patients with insulin-dependent CF-related diabetes ( CFRD ) ( 8 male , 1 female , mean age 21.9 years ) .
	manualset3
125161	12	404471	13	NULL	NULL	0	NULL	mean age 21.9 years 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A double-blind study was performed on 10 patients with type 1 diabetes mellitus ( DM ) without CF ( 3 male , 7 female , mean age 25.5 years ) and 9 patients with insulin-dependent CF-related diabetes ( CFRD ) ( 8 male , 1 female , mean age 21.9 years ) .
	manualset3
125162	1	404472	13	NULL	NULL	0	NULL	observations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our observations suggest that limb and tail defects observed in mice homozygous for the Repeated Epilation mutation may be secondary to primary changes occurring in the epidermis .
	manualset3
125163	2	404472	13	NULL	NULL	0	NULL	limb defects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our observations suggest that limb and tail defects observed in mice homozygous for the Repeated Epilation mutation may be secondary to primary changes occurring in the epidermis .
	manualset3
125164	3	404472	13	NULL	NULL	0	NULL	tail defects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our observations suggest that limb and tail defects observed in mice homozygous for the Repeated Epilation mutation may be secondary to primary changes occurring in the epidermis .
	manualset3
125165	4	404472	13	NULL	NULL	0	NULL	mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our observations suggest that limb and tail defects observed in mice homozygous for the Repeated Epilation mutation may be secondary to primary changes occurring in the epidermis .
	manualset3
125166	5	404472	13	NULL	NULL	0	NULL	Epilation mutation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our observations suggest that limb and tail defects observed in mice homozygous for the Repeated Epilation mutation may be secondary to primary changes occurring in the epidermis .
	manualset3
125167	6	404472	13	NULL	NULL	0	NULL	secondary changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our observations suggest that limb and tail defects observed in mice homozygous for the Repeated Epilation mutation may be secondary to primary changes occurring in the epidermis .
	manualset3
125168	7	404472	13	NULL	NULL	0	NULL	primary changes 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our observations suggest that limb and tail defects observed in mice homozygous for the Repeated Epilation mutation may be secondary to primary changes occurring in the epidermis .
	manualset3
125169	8	404472	13	NULL	NULL	0	NULL	epidermis 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our observations suggest that limb and tail defects observed in mice homozygous for the Repeated Epilation mutation may be secondary to primary changes occurring in the epidermis .
	manualset3
125170	1	404473	13	NULL	NULL	0	NULL	purpose	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our purpose was to review the literature concerning MIS THA , to determine if using short stems over standard femoral components is beneficial and if surgical approach affects the ability to use any type of stem .
	manualset3
125171	2	404473	13	NULL	NULL	0	NULL	literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our purpose was to review the literature concerning MIS THA , to determine if using short stems over standard femoral components is beneficial and if surgical approach affects the ability to use any type of stem .
	manualset3
125172	3	404473	13	NULL	NULL	0	NULL	MIS THA	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our purpose was to review the literature concerning MIS THA , to determine if using short stems over standard femoral components is beneficial and if surgical approach affects the ability to use any type of stem .
	manualset3
125173	4	404473	13	NULL	NULL	0	NULL	short stems	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our purpose was to review the literature concerning MIS THA , to determine if using short stems over standard femoral components is beneficial and if surgical approach affects the ability to use any type of stem .
	manualset3
125174	5	404473	13	NULL	NULL	0	NULL	femoral components	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our purpose was to review the literature concerning MIS THA , to determine if using short stems over standard femoral components is beneficial and if surgical approach affects the ability to use any type of stem .
	manualset3
125175	6	404473	13	NULL	NULL	0	NULL	surgical approach 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our purpose was to review the literature concerning MIS THA , to determine if using short stems over standard femoral components is beneficial and if surgical approach affects the ability to use any type of stem .
	manualset3
125176	7	404473	13	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our purpose was to review the literature concerning MIS THA , to determine if using short stems over standard femoral components is beneficial and if surgical approach affects the ability to use any type of stem .
	manualset3
125177	8	404473	13	NULL	NULL	0	NULL	type of stem	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our purpose was to review the literature concerning MIS THA , to determine if using short stems over standard femoral components is beneficial and if surgical approach affects the ability to use any type of stem .
	manualset3
125178	1	404474	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results are consistent with diazepam and allopregnanolone acting through the GABAA receptors of the MCG to enhance female sexual receptivity and with estradiol potentiating the effect of diazepam in the MCG to increase open-field behavior .
	manualset3
125179	2	404474	13	NULL	NULL	0	NULL	diazepam	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results are consistent with diazepam and allopregnanolone acting through the GABAA receptors of the MCG to enhance female sexual receptivity and with estradiol potentiating the effect of diazepam in the MCG to increase open-field behavior .
	manualset3
125180	3	404474	13	NULL	NULL	0	NULL	allopregnanolone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results are consistent with diazepam and allopregnanolone acting through the GABAA receptors of the MCG to enhance female sexual receptivity and with estradiol potentiating the effect of diazepam in the MCG to increase open-field behavior .
	manualset3
125181	4	404474	13	NULL	NULL	0	NULL	GABAA receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results are consistent with diazepam and allopregnanolone acting through the GABAA receptors of the MCG to enhance female sexual receptivity and with estradiol potentiating the effect of diazepam in the MCG to increase open-field behavior .
	manualset3
125182	5	404474	13	NULL	NULL	0	NULL	MCG	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results are consistent with diazepam and allopregnanolone acting through the GABAA receptors of the MCG to enhance female sexual receptivity and with estradiol potentiating the effect of diazepam in the MCG to increase open-field behavior .
	manualset3
125183	6	404474	13	NULL	NULL	0	NULL	female sexual receptivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results are consistent with diazepam and allopregnanolone acting through the GABAA receptors of the MCG to enhance female sexual receptivity and with estradiol potentiating the effect of diazepam in the MCG to increase open-field behavior .
	manualset3
125184	7	404474	13	NULL	NULL	0	NULL	estradiol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results are consistent with diazepam and allopregnanolone acting through the GABAA receptors of the MCG to enhance female sexual receptivity and with estradiol potentiating the effect of diazepam in the MCG to increase open-field behavior .
	manualset3
125185	8	404474	13	NULL	NULL	0	NULL	effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results are consistent with diazepam and allopregnanolone acting through the GABAA receptors of the MCG to enhance female sexual receptivity and with estradiol potentiating the effect of diazepam in the MCG to increase open-field behavior .
	manualset3
125186	9	404474	13	NULL	NULL	0	NULL	diazepam	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results are consistent with diazepam and allopregnanolone acting through the GABAA receptors of the MCG to enhance female sexual receptivity and with estradiol potentiating the effect of diazepam in the MCG to increase open-field behavior .
	manualset3
125187	10	404474	13	NULL	NULL	0	NULL	MCG 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results are consistent with diazepam and allopregnanolone acting through the GABAA receptors of the MCG to enhance female sexual receptivity and with estradiol potentiating the effect of diazepam in the MCG to increase open-field behavior .
	manualset3
125188	11	404474	13	NULL	NULL	0	NULL	open-field behavior	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results are consistent with diazepam and allopregnanolone acting through the GABAA receptors of the MCG to enhance female sexual receptivity and with estradiol potentiating the effect of diazepam in the MCG to increase open-field behavior .
	manualset3
125189	1	404475	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results are in agreement with the notion that this activity is localized at the plasma membrane and can be attributed to an O2 * -- synthesizing enzyme with catalytic and kinetic properties similar to that of the NADPH oxidase of mammalian phagocytes , with the important exception that it utilizes NADH instead of NADPH as electron donor .
	manualset3
125190	2	404475	13	NULL	NULL	0	NULL	agreement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results are in agreement with the notion that this activity is localized at the plasma membrane and can be attributed to an O2 * -- synthesizing enzyme with catalytic and kinetic properties similar to that of the NADPH oxidase of mammalian phagocytes , with the important exception that it utilizes NADH instead of NADPH as electron donor .
	manualset3
125191	3	404475	13	NULL	NULL	0	NULL	notion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results are in agreement with the notion that this activity is localized at the plasma membrane and can be attributed to an O2 * -- synthesizing enzyme with catalytic and kinetic properties similar to that of the NADPH oxidase of mammalian phagocytes , with the important exception that it utilizes NADH instead of NADPH as electron donor .
	manualset3
125192	4	404475	13	NULL	NULL	0	NULL	plasma membrane 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results are in agreement with the notion that this activity is localized at the plasma membrane and can be attributed to an O2 * -- synthesizing enzyme with catalytic and kinetic properties similar to that of the NADPH oxidase of mammalian phagocytes , with the important exception that it utilizes NADH instead of NADPH as electron donor .
	manualset3
125193	5	404475	13	NULL	NULL	0	NULL	O2 * -- synthesizing enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results are in agreement with the notion that this activity is localized at the plasma membrane and can be attributed to an O2 * -- synthesizing enzyme with catalytic and kinetic properties similar to that of the NADPH oxidase of mammalian phagocytes , with the important exception that it utilizes NADH instead of NADPH as electron donor .
	manualset3
125194	6	404475	13	NULL	NULL	0	NULL	catalytic properties	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results are in agreement with the notion that this activity is localized at the plasma membrane and can be attributed to an O2 * -- synthesizing enzyme with catalytic and kinetic properties similar to that of the NADPH oxidase of mammalian phagocytes , with the important exception that it utilizes NADH instead of NADPH as electron donor .
	manualset3
125195	7	404475	13	NULL	NULL	0	NULL	kinetic properties	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results are in agreement with the notion that this activity is localized at the plasma membrane and can be attributed to an O2 * -- synthesizing enzyme with catalytic and kinetic properties similar to that of the NADPH oxidase of mammalian phagocytes , with the important exception that it utilizes NADH instead of NADPH as electron donor .
	manualset3
125196	8	404475	13	NULL	NULL	0	NULL	NADPH oxidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results are in agreement with the notion that this activity is localized at the plasma membrane and can be attributed to an O2 * -- synthesizing enzyme with catalytic and kinetic properties similar to that of the NADPH oxidase of mammalian phagocytes , with the important exception that it utilizes NADH instead of NADPH as electron donor .
	manualset3
125197	9	404475	13	NULL	NULL	0	NULL	mammalian phagocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results are in agreement with the notion that this activity is localized at the plasma membrane and can be attributed to an O2 * -- synthesizing enzyme with catalytic and kinetic properties similar to that of the NADPH oxidase of mammalian phagocytes , with the important exception that it utilizes NADH instead of NADPH as electron donor .
	manualset3
125198	10	404475	13	NULL	NULL	0	NULL	exception 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results are in agreement with the notion that this activity is localized at the plasma membrane and can be attributed to an O2 * -- synthesizing enzyme with catalytic and kinetic properties similar to that of the NADPH oxidase of mammalian phagocytes , with the important exception that it utilizes NADH instead of NADPH as electron donor .
	manualset3
125199	11	404475	13	NULL	NULL	NULL	NULL	NADH	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our results are in agreement with the notion that this activity is localized at the plasma membrane and can be attributed to an O2 * -- synthesizing enzyme with catalytic and kinetic properties similar to that of the NADPH oxidase of mammalian phagocytes , with the important exception that it utilizes NADH instead of NADPH as electron donor .
	manualset3
125200	12	404475	13	NULL	NULL	NULL	NULL	NADPH	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our results are in agreement with the notion that this activity is localized at the plasma membrane and can be attributed to an O2 * -- synthesizing enzyme with catalytic and kinetic properties similar to that of the NADPH oxidase of mammalian phagocytes , with the important exception that it utilizes NADH instead of NADPH as electron donor .
	manualset3
125201	13	404475	13	NULL	NULL	NULL	NULL	electron donor	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our results are in agreement with the notion that this activity is localized at the plasma membrane and can be attributed to an O2 * -- synthesizing enzyme with catalytic and kinetic properties similar to that of the NADPH oxidase of mammalian phagocytes , with the important exception that it utilizes NADH instead of NADPH as electron donor .
	manualset3
125202	1	404476	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results can be interpreted to indicate that alteration to voltage operated , felodipine-sensitive , calcium channels as well as , cadmium-sensitive sites contribute to the changes observed in the functional behavior of pulmonary blood vessels from pulmonary hypertensive rats .
	manualset3
125203	2	404476	13	NULL	NULL	0	NULL	alteration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results can be interpreted to indicate that alteration to voltage operated , felodipine-sensitive , calcium channels as well as , cadmium-sensitive sites contribute to the changes observed in the functional behavior of pulmonary blood vessels from pulmonary hypertensive rats .
	manualset3
125204	3	404476	13	NULL	NULL	0	NULL	voltage	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results can be interpreted to indicate that alteration to voltage operated , felodipine-sensitive , calcium channels as well as , cadmium-sensitive sites contribute to the changes observed in the functional behavior of pulmonary blood vessels from pulmonary hypertensive rats .
	manualset3
125205	4	404476	13	NULL	NULL	0	NULL	calcium channels	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results can be interpreted to indicate that alteration to voltage operated , felodipine-sensitive , calcium channels as well as , cadmium-sensitive sites contribute to the changes observed in the functional behavior of pulmonary blood vessels from pulmonary hypertensive rats .
	manualset3
125206	5	404476	13	NULL	NULL	0	NULL	cadmium-sensitive sites	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results can be interpreted to indicate that alteration to voltage operated , felodipine-sensitive , calcium channels as well as , cadmium-sensitive sites contribute to the changes observed in the functional behavior of pulmonary blood vessels from pulmonary hypertensive rats .
	manualset3
125207	6	404476	13	NULL	NULL	0	NULL	changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results can be interpreted to indicate that alteration to voltage operated , felodipine-sensitive , calcium channels as well as , cadmium-sensitive sites contribute to the changes observed in the functional behavior of pulmonary blood vessels from pulmonary hypertensive rats .
	manualset3
125208	7	404476	13	NULL	NULL	0	NULL	functional behavior	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results can be interpreted to indicate that alteration to voltage operated , felodipine-sensitive , calcium channels as well as , cadmium-sensitive sites contribute to the changes observed in the functional behavior of pulmonary blood vessels from pulmonary hypertensive rats .
	manualset3
125209	8	404476	13	NULL	NULL	0	NULL	pulmonary blood vessels 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results can be interpreted to indicate that alteration to voltage operated , felodipine-sensitive , calcium channels as well as , cadmium-sensitive sites contribute to the changes observed in the functional behavior of pulmonary blood vessels from pulmonary hypertensive rats .
	manualset3
125210	9	404476	13	NULL	NULL	0	NULL	pulmonary hypertensive rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results can be interpreted to indicate that alteration to voltage operated , felodipine-sensitive , calcium channels as well as , cadmium-sensitive sites contribute to the changes observed in the functional behavior of pulmonary blood vessels from pulmonary hypertensive rats .
	manualset3
125211	1	404477	13	NULL	NULL	0	NULL	double molar quantity 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A double molar quantity of boronic acid led , for both 2-deoxy-hexoses , to the diester of the open-chain aldehydo isomer as the major product : the 3 , 5 : 4 , 6 - diester for the lyxo-configured deoxy-hexose , and the 3 , 4 : 5 , 6 - diester of the arabino-configured isomer .
	manualset3
125212	2	404477	13	NULL	NULL	0	NULL	boronic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A double molar quantity of boronic acid led , for both 2-deoxy-hexoses , to the diester of the open-chain aldehydo isomer as the major product : the 3 , 5 : 4 , 6 - diester for the lyxo-configured deoxy-hexose , and the 3 , 4 : 5 , 6 - diester of the arabino-configured isomer .
	manualset3
125213	3	404477	13	NULL	NULL	0	NULL	2-deoxy-hexoses	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A double molar quantity of boronic acid led , for both 2-deoxy-hexoses , to the diester of the open-chain aldehydo isomer as the major product : the 3 , 5 : 4 , 6 - diester for the lyxo-configured deoxy-hexose , and the 3 , 4 : 5 , 6 - diester of the arabino-configured isomer .
	manualset3
125214	4	404477	13	NULL	NULL	0	NULL	diester	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A double molar quantity of boronic acid led , for both 2-deoxy-hexoses , to the diester of the open-chain aldehydo isomer as the major product : the 3 , 5 : 4 , 6 - diester for the lyxo-configured deoxy-hexose , and the 3 , 4 : 5 , 6 - diester of the arabino-configured isomer .
	manualset3
125215	5	404477	13	NULL	NULL	0	NULL	open-chain aldehydo isomer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A double molar quantity of boronic acid led , for both 2-deoxy-hexoses , to the diester of the open-chain aldehydo isomer as the major product : the 3 , 5 : 4 , 6 - diester for the lyxo-configured deoxy-hexose , and the 3 , 4 : 5 , 6 - diester of the arabino-configured isomer .
	manualset3
125216	6	404477	13	NULL	NULL	0	NULL	major product	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A double molar quantity of boronic acid led , for both 2-deoxy-hexoses , to the diester of the open-chain aldehydo isomer as the major product : the 3 , 5 : 4 , 6 - diester for the lyxo-configured deoxy-hexose , and the 3 , 4 : 5 , 6 - diester of the arabino-configured isomer .
	manualset3
125217	7	404477	13	NULL	NULL	0	NULL	3 , 5 : 4 , 6 - diester 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A double molar quantity of boronic acid led , for both 2-deoxy-hexoses , to the diester of the open-chain aldehydo isomer as the major product : the 3 , 5 : 4 , 6 - diester for the lyxo-configured deoxy-hexose , and the 3 , 4 : 5 , 6 - diester of the arabino-configured isomer .
	manualset3
125218	8	404477	13	NULL	NULL	0	NULL	lyxo-configured deoxy-hexose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A double molar quantity of boronic acid led , for both 2-deoxy-hexoses , to the diester of the open-chain aldehydo isomer as the major product : the 3 , 5 : 4 , 6 - diester for the lyxo-configured deoxy-hexose , and the 3 , 4 : 5 , 6 - diester of the arabino-configured isomer .
	manualset3
125219	9	404477	13	NULL	NULL	0	NULL	3 , 4 : 5 , 6 - diester	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A double molar quantity of boronic acid led , for both 2-deoxy-hexoses , to the diester of the open-chain aldehydo isomer as the major product : the 3 , 5 : 4 , 6 - diester for the lyxo-configured deoxy-hexose , and the 3 , 4 : 5 , 6 - diester of the arabino-configured isomer .
	manualset3
125220	10	404477	13	NULL	NULL	0	NULL	arabino-configured isomer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A double molar quantity of boronic acid led , for both 2-deoxy-hexoses , to the diester of the open-chain aldehydo isomer as the major product : the 3 , 5 : 4 , 6 - diester for the lyxo-configured deoxy-hexose , and the 3 , 4 : 5 , 6 - diester of the arabino-configured isomer .
	manualset3
125221	1	404478	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results corroborate the leading role of the T and Haarlem genotypes in the epidemiology of drug-resistant TB in Poland .
	manualset3
125222	2	404478	13	NULL	NULL	0	NULL	role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results corroborate the leading role of the T and Haarlem genotypes in the epidemiology of drug-resistant TB in Poland .
	manualset3
125223	3	404478	13	NULL	NULL	0	NULL	T genotypes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results corroborate the leading role of the T and Haarlem genotypes in the epidemiology of drug-resistant TB in Poland .
	manualset3
125224	4	404478	13	NULL	NULL	0	NULL	Haarlem genotypes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results corroborate the leading role of the T and Haarlem genotypes in the epidemiology of drug-resistant TB in Poland .
	manualset3
125225	5	404478	13	NULL	NULL	0	NULL	epidemiology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results corroborate the leading role of the T and Haarlem genotypes in the epidemiology of drug-resistant TB in Poland .
	manualset3
125226	6	404478	13	NULL	NULL	0	NULL	drug-resistant TB	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results corroborate the leading role of the T and Haarlem genotypes in the epidemiology of drug-resistant TB in Poland .
	manualset3
125227	7	404478	13	NULL	NULL	0	NULL	Poland	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results corroborate the leading role of the T and Haarlem genotypes in the epidemiology of drug-resistant TB in Poland .
	manualset3
125228	1	404479	13	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that ( 1 ) CD103 is upregulated on CD8 ( + ) T cells subsequent to their entry into the small intestinal epithelium , and ( 2 ) that the chemokine CCL25 enhances CD103-mediated adhesion to E-cadherin .
	manualset3
125229	2	404479	13	NULL	NULL	0	NULL	CD103	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that ( 1 ) CD103 is upregulated on CD8 ( + ) T cells subsequent to their entry into the small intestinal epithelium , and ( 2 ) that the chemokine CCL25 enhances CD103-mediated adhesion to E-cadherin .
	manualset3
125230	3	404479	13	NULL	NULL	0	NULL	CD8 ( + ) T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that ( 1 ) CD103 is upregulated on CD8 ( + ) T cells subsequent to their entry into the small intestinal epithelium , and ( 2 ) that the chemokine CCL25 enhances CD103-mediated adhesion to E-cadherin .
	manualset3
125231	4	404479	13	NULL	NULL	0	NULL	entry	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that ( 1 ) CD103 is upregulated on CD8 ( + ) T cells subsequent to their entry into the small intestinal epithelium , and ( 2 ) that the chemokine CCL25 enhances CD103-mediated adhesion to E-cadherin .
	manualset3
125232	5	404479	13	NULL	NULL	0	NULL	small intestinal epithelium 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that ( 1 ) CD103 is upregulated on CD8 ( + ) T cells subsequent to their entry into the small intestinal epithelium , and ( 2 ) that the chemokine CCL25 enhances CD103-mediated adhesion to E-cadherin .
	manualset3
125233	6	404479	13	NULL	NULL	0	NULL	chemokine CCL25	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that ( 1 ) CD103 is upregulated on CD8 ( + ) T cells subsequent to their entry into the small intestinal epithelium , and ( 2 ) that the chemokine CCL25 enhances CD103-mediated adhesion to E-cadherin .
	manualset3
125234	7	404479	13	NULL	NULL	0	NULL	CD103-mediated adhesion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that ( 1 ) CD103 is upregulated on CD8 ( + ) T cells subsequent to their entry into the small intestinal epithelium , and ( 2 ) that the chemokine CCL25 enhances CD103-mediated adhesion to E-cadherin .
	manualset3
125235	8	404479	13	NULL	NULL	0	NULL	E-cadherin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that ( 1 ) CD103 is upregulated on CD8 ( + ) T cells subsequent to their entry into the small intestinal epithelium , and ( 2 ) that the chemokine CCL25 enhances CD103-mediated adhesion to E-cadherin .
	manualset3
125236	1	404480	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that Acivicin is also an inhibitor of de novo pyrimidine biosynthesis .
	manualset3
125237	2	404480	13	NULL	NULL	0	NULL	Acivicin 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that Acivicin is also an inhibitor of de novo pyrimidine biosynthesis .
	manualset3
125238	3	404480	13	NULL	NULL	0	NULL	inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that Acivicin is also an inhibitor of de novo pyrimidine biosynthesis .
	manualset3
125239	4	404480	13	NULL	NULL	0	NULL	de novo pyrimidine biosynthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that Acivicin is also an inhibitor of de novo pyrimidine biosynthesis .
	manualset3
125262	1	404481	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that MMP-9 is crucially involved in radiation-enhanced LLC-LM cell invasiveness in vitro and in pulmonary metastasis from inadequately irradiated primary tumor in vivo .
	manualset3
125263	2	404481	13	NULL	NULL	0	NULL	MMP-9	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that MMP-9 is crucially involved in radiation-enhanced LLC-LM cell invasiveness in vitro and in pulmonary metastasis from inadequately irradiated primary tumor in vivo .
	manualset3
125264	3	404481	13	NULL	NULL	0	NULL	LLC-LM cell invasiveness	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that MMP-9 is crucially involved in radiation-enhanced LLC-LM cell invasiveness in vitro and in pulmonary metastasis from inadequately irradiated primary tumor in vivo .
	manualset3
125265	4	404481	13	NULL	NULL	0	NULL	pulmonary metastasis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that MMP-9 is crucially involved in radiation-enhanced LLC-LM cell invasiveness in vitro and in pulmonary metastasis from inadequately irradiated primary tumor in vivo .
	manualset3
125266	5	404481	13	NULL	NULL	0	NULL	primary tumor 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that MMP-9 is crucially involved in radiation-enhanced LLC-LM cell invasiveness in vitro and in pulmonary metastasis from inadequately irradiated primary tumor in vivo .
	manualset3
125267	1	404482	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that Ras - and Rac1-mediated p38 and JNK signals are required for Stat3 transcriptional activity induced by the Src oncoprotein .
	manualset3
125268	2	404482	13	NULL	NULL	0	NULL	Ras -mediated p38 signals 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that Ras - and Rac1-mediated p38 and JNK signals are required for Stat3 transcriptional activity induced by the Src oncoprotein .
	manualset3
125269	3	404482	13	NULL	NULL	0	NULL	Ras -mediated JNK signals	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that Ras - and Rac1-mediated p38 and JNK signals are required for Stat3 transcriptional activity induced by the Src oncoprotein .
	manualset3
125270	4	404482	13	NULL	NULL	0	NULL	Rac1-mediated p38 signals	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that Ras - and Rac1-mediated p38 and JNK signals are required for Stat3 transcriptional activity induced by the Src oncoprotein .
	manualset3
125271	5	404482	13	NULL	NULL	0	NULL	Rac1-mediated JNK signals 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that Ras - and Rac1-mediated p38 and JNK signals are required for Stat3 transcriptional activity induced by the Src oncoprotein .
	manualset3
125272	6	404482	13	NULL	NULL	0	NULL	Stat3 transcriptional activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that Ras - and Rac1-mediated p38 and JNK signals are required for Stat3 transcriptional activity induced by the Src oncoprotein .
	manualset3
125273	7	404482	13	NULL	NULL	0	NULL	Src oncoprotein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that Ras - and Rac1-mediated p38 and JNK signals are required for Stat3 transcriptional activity induced by the Src oncoprotein .
	manualset3
125274	1	404483	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that TCS arises from haploinsufficiency of a protein that plays a crucial role in craniofacial development and indicate that correct dosage of treacle is essential for survival of cephalic neural crest cells .
	manualset3
125275	2	404483	13	NULL	NULL	0	NULL	TCS 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that TCS arises from haploinsufficiency of a protein that plays a crucial role in craniofacial development and indicate that correct dosage of treacle is essential for survival of cephalic neural crest cells .
	manualset3
125276	3	404483	13	NULL	NULL	0	NULL	haploinsufficiency	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that TCS arises from haploinsufficiency of a protein that plays a crucial role in craniofacial development and indicate that correct dosage of treacle is essential for survival of cephalic neural crest cells .
	manualset3
125277	4	404483	13	NULL	NULL	0	NULL	protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that TCS arises from haploinsufficiency of a protein that plays a crucial role in craniofacial development and indicate that correct dosage of treacle is essential for survival of cephalic neural crest cells .
	manualset3
125278	5	404483	13	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that TCS arises from haploinsufficiency of a protein that plays a crucial role in craniofacial development and indicate that correct dosage of treacle is essential for survival of cephalic neural crest cells .
	manualset3
125279	6	404483	13	NULL	NULL	0	NULL	 craniofacial development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that TCS arises from haploinsufficiency of a protein that plays a crucial role in craniofacial development and indicate that correct dosage of treacle is essential for survival of cephalic neural crest cells .
	manualset3
125280	7	404483	13	NULL	NULL	0	NULL	dosage	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that TCS arises from haploinsufficiency of a protein that plays a crucial role in craniofacial development and indicate that correct dosage of treacle is essential for survival of cephalic neural crest cells .
	manualset3
125281	8	404483	13	NULL	NULL	0	NULL	treacle	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that TCS arises from haploinsufficiency of a protein that plays a crucial role in craniofacial development and indicate that correct dosage of treacle is essential for survival of cephalic neural crest cells .
	manualset3
125282	9	404483	13	NULL	NULL	0	NULL	survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that TCS arises from haploinsufficiency of a protein that plays a crucial role in craniofacial development and indicate that correct dosage of treacle is essential for survival of cephalic neural crest cells .
	manualset3
125283	10	404483	13	NULL	NULL	0	NULL	cephalic neural crest cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that TCS arises from haploinsufficiency of a protein that plays a crucial role in craniofacial development and indicate that correct dosage of treacle is essential for survival of cephalic neural crest cells .
	manualset3
125284	1	404484	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that expression of neuropeptide tyrosine , one of the most abundant and widespread peptides in the mammalian nervous system , occurs in non-neuronal cells , in keeping with the emerging view that neuropeptide synthesis is not restricted to cells of the nervous system .
	manualset3
125285	2	404484	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that expression of neuropeptide tyrosine , one of the most abundant and widespread peptides in the mammalian nervous system , occurs in non-neuronal cells , in keeping with the emerging view that neuropeptide synthesis is not restricted to cells of the nervous system .
	manualset3
125286	3	404484	13	NULL	NULL	0	NULL	neuropeptide tyrosine	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that expression of neuropeptide tyrosine , one of the most abundant and widespread peptides in the mammalian nervous system , occurs in non-neuronal cells , in keeping with the emerging view that neuropeptide synthesis is not restricted to cells of the nervous system .
	manualset3
125287	4	404484	13	NULL	NULL	0	NULL	peptides 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that expression of neuropeptide tyrosine , one of the most abundant and widespread peptides in the mammalian nervous system , occurs in non-neuronal cells , in keeping with the emerging view that neuropeptide synthesis is not restricted to cells of the nervous system .
	manualset3
125288	5	404484	13	NULL	NULL	0	NULL	mammalian nervous system 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that expression of neuropeptide tyrosine , one of the most abundant and widespread peptides in the mammalian nervous system , occurs in non-neuronal cells , in keeping with the emerging view that neuropeptide synthesis is not restricted to cells of the nervous system .
	manualset3
125289	6	404484	13	NULL	NULL	0	NULL	non-neuronal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that expression of neuropeptide tyrosine , one of the most abundant and widespread peptides in the mammalian nervous system , occurs in non-neuronal cells , in keeping with the emerging view that neuropeptide synthesis is not restricted to cells of the nervous system .
	manualset3
125290	7	404484	13	NULL	NULL	0	NULL	view	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that expression of neuropeptide tyrosine , one of the most abundant and widespread peptides in the mammalian nervous system , occurs in non-neuronal cells , in keeping with the emerging view that neuropeptide synthesis is not restricted to cells of the nervous system .
	manualset3
125291	8	404484	13	NULL	NULL	0	NULL	neuropeptide synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that expression of neuropeptide tyrosine , one of the most abundant and widespread peptides in the mammalian nervous system , occurs in non-neuronal cells , in keeping with the emerging view that neuropeptide synthesis is not restricted to cells of the nervous system .
	manualset3
125292	9	404484	13	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that expression of neuropeptide tyrosine , one of the most abundant and widespread peptides in the mammalian nervous system , occurs in non-neuronal cells , in keeping with the emerging view that neuropeptide synthesis is not restricted to cells of the nervous system .
	manualset3
125293	10	404484	13	NULL	NULL	0	NULL	nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that expression of neuropeptide tyrosine , one of the most abundant and widespread peptides in the mammalian nervous system , occurs in non-neuronal cells , in keeping with the emerging view that neuropeptide synthesis is not restricted to cells of the nervous system .
	manualset3
125294	1	404485	13	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that osthole may be just as effective as 17beta-estradiol in suppressing bone loss due to ovariectomy but osthole perhaps does not work through the estrogen pathway .
	manualset3
125295	2	404485	13	NULL	NULL	0	NULL	osthole	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that osthole may be just as effective as 17beta-estradiol in suppressing bone loss due to ovariectomy but osthole perhaps does not work through the estrogen pathway .
	manualset3
125296	3	404485	13	NULL	NULL	0	NULL	17beta-estradiol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that osthole may be just as effective as 17beta-estradiol in suppressing bone loss due to ovariectomy but osthole perhaps does not work through the estrogen pathway .
	manualset3
125297	4	404485	13	NULL	NULL	0	NULL	bone loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that osthole may be just as effective as 17beta-estradiol in suppressing bone loss due to ovariectomy but osthole perhaps does not work through the estrogen pathway .
	manualset3
125298	5	404485	13	NULL	NULL	0	NULL	ovariectomy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that osthole may be just as effective as 17beta-estradiol in suppressing bone loss due to ovariectomy but osthole perhaps does not work through the estrogen pathway .
	manualset3
125299	6	404485	13	NULL	NULL	0	NULL	osthole	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that osthole may be just as effective as 17beta-estradiol in suppressing bone loss due to ovariectomy but osthole perhaps does not work through the estrogen pathway .
	manualset3
125300	7	404485	13	NULL	NULL	0	NULL	estrogen pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that osthole may be just as effective as 17beta-estradiol in suppressing bone loss due to ovariectomy but osthole perhaps does not work through the estrogen pathway .
	manualset3
125301	1	404486	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that the production of cyanobacterial hepatotoxins in lichen symbiosis is a global phenomenon and occurs in many different lichen lineages .
	manualset3
125302	2	404486	13	NULL	NULL	0	NULL	production 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that the production of cyanobacterial hepatotoxins in lichen symbiosis is a global phenomenon and occurs in many different lichen lineages .
	manualset3
125303	3	404486	13	NULL	NULL	0	NULL	cyanobacterial hepatotoxins	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that the production of cyanobacterial hepatotoxins in lichen symbiosis is a global phenomenon and occurs in many different lichen lineages .
	manualset3
125304	4	404486	13	NULL	NULL	0	NULL	lichen symbiosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that the production of cyanobacterial hepatotoxins in lichen symbiosis is a global phenomenon and occurs in many different lichen lineages .
	manualset3
125305	5	404486	13	NULL	NULL	0	NULL	global phenomenon	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that the production of cyanobacterial hepatotoxins in lichen symbiosis is a global phenomenon and occurs in many different lichen lineages .
	manualset3
125306	6	404486	13	NULL	NULL	0	NULL	lichen lineages	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that the production of cyanobacterial hepatotoxins in lichen symbiosis is a global phenomenon and occurs in many different lichen lineages .
	manualset3
125307	1	404487	13	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that these microspheres can be successfully employed for simultaneous cellular labeling and controlled transfer of various cargos such as fluorophores , proteins and nucleic acids into ES cells without any significant toxicity or loss of pluripotency .
	manualset3
125308	2	404487	13	NULL	NULL	0	NULL	microspheres	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that these microspheres can be successfully employed for simultaneous cellular labeling and controlled transfer of various cargos such as fluorophores , proteins and nucleic acids into ES cells without any significant toxicity or loss of pluripotency .
	manualset3
125309	3	404487	13	NULL	NULL	NULL	NULL	transfer	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that these microspheres can be successfully employed for simultaneous cellular labeling and controlled transfer of various cargos such as fluorophores , proteins and nucleic acids into ES cells without any significant toxicity or loss of pluripotency .
	manualset3
125313	4	404487	13	NULL	NULL	0	NULL	cargos 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that these microspheres can be successfully employed for simultaneous cellular labeling and controlled transfer of various cargos such as fluorophores , proteins and nucleic acids into ES cells without any significant toxicity or loss of pluripotency .
	manualset3
125314	5	404487	13	NULL	NULL	0	NULL	fluorophores	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that these microspheres can be successfully employed for simultaneous cellular labeling and controlled transfer of various cargos such as fluorophores , proteins and nucleic acids into ES cells without any significant toxicity or loss of pluripotency .
	manualset3
125315	6	404487	13	NULL	NULL	0	NULL	proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that these microspheres can be successfully employed for simultaneous cellular labeling and controlled transfer of various cargos such as fluorophores , proteins and nucleic acids into ES cells without any significant toxicity or loss of pluripotency .
	manualset3
125316	7	404487	13	NULL	NULL	0	NULL	nucleic acids	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that these microspheres can be successfully employed for simultaneous cellular labeling and controlled transfer of various cargos such as fluorophores , proteins and nucleic acids into ES cells without any significant toxicity or loss of pluripotency .
	manualset3
125317	8	404487	13	NULL	NULL	0	NULL	ES cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that these microspheres can be successfully employed for simultaneous cellular labeling and controlled transfer of various cargos such as fluorophores , proteins and nucleic acids into ES cells without any significant toxicity or loss of pluripotency .
	manualset3
125318	9	404487	13	NULL	NULL	0	NULL	toxicity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that these microspheres can be successfully employed for simultaneous cellular labeling and controlled transfer of various cargos such as fluorophores , proteins and nucleic acids into ES cells without any significant toxicity or loss of pluripotency .
	manualset3
125319	10	404487	13	NULL	NULL	0	NULL	loss of pluripotency	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate that these microspheres can be successfully employed for simultaneous cellular labeling and controlled transfer of various cargos such as fluorophores , proteins and nucleic acids into ES cells without any significant toxicity or loss of pluripotency .
	manualset3
125322	1	404488	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the feasibility of engineering magnetism at visible frequencies and pave the way towards magnetic and left-handed components for visible optics .
	manualset3
125323	2	404488	13	NULL	NULL	0	NULL	feasibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the feasibility of engineering magnetism at visible frequencies and pave the way towards magnetic and left-handed components for visible optics .
	manualset3
125325	3	404488	13	NULL	NULL	0	NULL	engineering magnetism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the feasibility of engineering magnetism at visible frequencies and pave the way towards magnetic and left-handed components for visible optics .
	manualset3
125326	4	404488	13	NULL	NULL	0	NULL	visible frequencies 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the feasibility of engineering magnetism at visible frequencies and pave the way towards magnetic and left-handed components for visible optics .
	manualset3
125329	5	404488	13	NULL	NULL	0	NULL	magnetic components	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the feasibility of engineering magnetism at visible frequencies and pave the way towards magnetic and left-handed components for visible optics .
	manualset3
125330	6	404488	13	NULL	NULL	0	NULL	left-handed components 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the feasibility of engineering magnetism at visible frequencies and pave the way towards magnetic and left-handed components for visible optics .
	manualset3
125332	7	404488	13	NULL	NULL	0	NULL	visible optics 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the feasibility of engineering magnetism at visible frequencies and pave the way towards magnetic and left-handed components for visible optics .
	manualset3
125334	1	404489	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the power of C. elegans embryogenesis as a model to dissect the interaction between differentiation and proliferation , and an effective approach combining genetic and statistical analysis at single-cell resolution .
	manualset3
125335	2	404489	13	NULL	NULL	0	NULL	power	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the power of C. elegans embryogenesis as a model to dissect the interaction between differentiation and proliferation , and an effective approach combining genetic and statistical analysis at single-cell resolution .
	manualset3
125336	3	404489	13	NULL	NULL	0	NULL	C. elegans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the power of C. elegans embryogenesis as a model to dissect the interaction between differentiation and proliferation , and an effective approach combining genetic and statistical analysis at single-cell resolution .
	manualset3
125337	4	404489	13	NULL	NULL	0	NULL	embryogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the power of C. elegans embryogenesis as a model to dissect the interaction between differentiation and proliferation , and an effective approach combining genetic and statistical analysis at single-cell resolution .
	manualset3
125338	5	404489	13	NULL	NULL	0	NULL	model	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the power of C. elegans embryogenesis as a model to dissect the interaction between differentiation and proliferation , and an effective approach combining genetic and statistical analysis at single-cell resolution .
	manualset3
125339	6	404489	13	NULL	NULL	0	NULL	interaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the power of C. elegans embryogenesis as a model to dissect the interaction between differentiation and proliferation , and an effective approach combining genetic and statistical analysis at single-cell resolution .
	manualset3
125340	7	404489	13	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the power of C. elegans embryogenesis as a model to dissect the interaction between differentiation and proliferation , and an effective approach combining genetic and statistical analysis at single-cell resolution .
	manualset3
125341	8	404489	13	NULL	NULL	0	NULL	proliferation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the power of C. elegans embryogenesis as a model to dissect the interaction between differentiation and proliferation , and an effective approach combining genetic and statistical analysis at single-cell resolution .
	manualset3
125342	9	404489	13	NULL	NULL	0	NULL	effective approach 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the power of C. elegans embryogenesis as a model to dissect the interaction between differentiation and proliferation , and an effective approach combining genetic and statistical analysis at single-cell resolution .
	manualset3
125343	10	404489	13	NULL	NULL	0	NULL	genetic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the power of C. elegans embryogenesis as a model to dissect the interaction between differentiation and proliferation , and an effective approach combining genetic and statistical analysis at single-cell resolution .
	manualset3
125344	11	404489	13	NULL	NULL	0	NULL	statistical analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the power of C. elegans embryogenesis as a model to dissect the interaction between differentiation and proliferation , and an effective approach combining genetic and statistical analysis at single-cell resolution .
	manualset3
125345	12	404489	13	NULL	NULL	0	NULL	single-cell resolution	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the power of C. elegans embryogenesis as a model to dissect the interaction between differentiation and proliferation , and an effective approach combining genetic and statistical analysis at single-cell resolution .
	manualset3
125346	1	404490	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the promises and limitations for rational design to obtain high level expression and secretion of heterologous proteins by S. cerevisiae .
	manualset3
125347	2	404490	13	NULL	NULL	0	NULL	promises	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the promises and limitations for rational design to obtain high level expression and secretion of heterologous proteins by S. cerevisiae .
	manualset3
125348	3	404490	13	NULL	NULL	0	NULL	limitations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the promises and limitations for rational design to obtain high level expression and secretion of heterologous proteins by S. cerevisiae .
	manualset3
125349	4	404490	13	NULL	NULL	0	NULL	rational design	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the promises and limitations for rational design to obtain high level expression and secretion of heterologous proteins by S. cerevisiae .
	manualset3
125350	5	404490	13	NULL	NULL	0	NULL	level 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the promises and limitations for rational design to obtain high level expression and secretion of heterologous proteins by S. cerevisiae .
	manualset3
125351	6	404490	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the promises and limitations for rational design to obtain high level expression and secretion of heterologous proteins by S. cerevisiae .
	manualset3
125352	7	404490	13	NULL	NULL	0	NULL	secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the promises and limitations for rational design to obtain high level expression and secretion of heterologous proteins by S. cerevisiae .
	manualset3
125353	8	404490	13	NULL	NULL	0	NULL	heterologous proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the promises and limitations for rational design to obtain high level expression and secretion of heterologous proteins by S. cerevisiae .
	manualset3
125354	9	404490	13	NULL	NULL	0	NULL	S. cerevisiae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the promises and limitations for rational design to obtain high level expression and secretion of heterologous proteins by S. cerevisiae .
	manualset3
125541	1	404491	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the relationship between TGF-beta ( 1 ) concentrations and HIV infection advancement with marked elevation in the late stages of the disease .
	manualset3
125557	2	404491	13	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the relationship between TGF-beta ( 1 ) concentrations and HIV infection advancement with marked elevation in the late stages of the disease .
	manualset3
125558	3	404491	13	NULL	NULL	0	NULL	TGF-beta ( 1 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the relationship between TGF-beta ( 1 ) concentrations and HIV infection advancement with marked elevation in the late stages of the disease .
	manualset3
125559	4	404491	13	NULL	NULL	0	NULL	concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the relationship between TGF-beta ( 1 ) concentrations and HIV infection advancement with marked elevation in the late stages of the disease .
	manualset3
125560	5	404491	13	NULL	NULL	0	NULL	HIV infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the relationship between TGF-beta ( 1 ) concentrations and HIV infection advancement with marked elevation in the late stages of the disease .
	manualset3
125561	6	404491	13	NULL	NULL	0	NULL	advancement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the relationship between TGF-beta ( 1 ) concentrations and HIV infection advancement with marked elevation in the late stages of the disease .
	manualset3
125562	7	404491	13	NULL	NULL	0	NULL	elevation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the relationship between TGF-beta ( 1 ) concentrations and HIV infection advancement with marked elevation in the late stages of the disease .
	manualset3
125563	8	404491	13	NULL	NULL	0	NULL	late stages	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the relationship between TGF-beta ( 1 ) concentrations and HIV infection advancement with marked elevation in the late stages of the disease .
	manualset3
125564	9	404491	13	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the relationship between TGF-beta ( 1 ) concentrations and HIV infection advancement with marked elevation in the late stages of the disease .
	manualset3
125565	1	404492	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the role of presynaptic mGluRs in the physiological control of movement for the first time .
	manualset3
125566	2	404492	13	NULL	NULL	0	NULL	role 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the role of presynaptic mGluRs in the physiological control of movement for the first time .
	manualset3
125567	3	404492	13	NULL	NULL	0	NULL	presynaptic mGluRs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the role of presynaptic mGluRs in the physiological control of movement for the first time .
	manualset3
125568	4	404492	13	NULL	NULL	0	NULL	physiological control	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the role of presynaptic mGluRs in the physiological control of movement for the first time .
	manualset3
125569	5	404492	13	NULL	NULL	0	NULL	movement 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the role of presynaptic mGluRs in the physiological control of movement for the first time .
	manualset3
125571	6	404492	13	NULL	NULL	0	NULL	first time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results demonstrate the role of presynaptic mGluRs in the physiological control of movement for the first time .
	manualset3
125572	1	404493	13	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results highlight the important role of L4 and L22 in ribosome function and assembly , and indicate that a variety of changes in these proteins can mediate macrolide resistance .
	manualset3
125573	2	404493	13	NULL	NULL	0	NULL	highlight	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results highlight the important role of L4 and L22 in ribosome function and assembly , and indicate that a variety of changes in these proteins can mediate macrolide resistance .
	manualset3
125574	3	404493	13	NULL	NULL	0	NULL	important role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results highlight the important role of L4 and L22 in ribosome function and assembly , and indicate that a variety of changes in these proteins can mediate macrolide resistance .
	manualset3
125575	4	404493	13	NULL	NULL	0	NULL	L4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results highlight the important role of L4 and L22 in ribosome function and assembly , and indicate that a variety of changes in these proteins can mediate macrolide resistance .
	manualset3
125576	5	404493	13	NULL	NULL	0	NULL	L22	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results highlight the important role of L4 and L22 in ribosome function and assembly , and indicate that a variety of changes in these proteins can mediate macrolide resistance .
	manualset3
125577	6	404493	13	NULL	NULL	0	NULL	ribosome function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results highlight the important role of L4 and L22 in ribosome function and assembly , and indicate that a variety of changes in these proteins can mediate macrolide resistance .
	manualset3
125578	7	404493	13	NULL	NULL	0	NULL	assembly	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results highlight the important role of L4 and L22 in ribosome function and assembly , and indicate that a variety of changes in these proteins can mediate macrolide resistance .
	manualset3
125579	8	404493	13	NULL	NULL	0	NULL	variety of changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results highlight the important role of L4 and L22 in ribosome function and assembly , and indicate that a variety of changes in these proteins can mediate macrolide resistance .
	manualset3
125581	9	404493	13	NULL	NULL	0	NULL	proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results highlight the important role of L4 and L22 in ribosome function and assembly , and indicate that a variety of changes in these proteins can mediate macrolide resistance .
	manualset3
125582	10	404493	13	NULL	NULL	0	NULL	macrolide resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results highlight the important role of L4 and L22 in ribosome function and assembly , and indicate that a variety of changes in these proteins can mediate macrolide resistance .
	manualset3
125583	1	404494	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results implicate that there is a functional relationship between glomerular filtration and urinary EGF excretion , and that the urinary EGF/Cr may be a reliable indicator of urinary EGF excretion in children with CRF .
	manualset3
125584	2	404494	13	NULL	NULL	0	NULL	relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results implicate that there is a functional relationship between glomerular filtration and urinary EGF excretion , and that the urinary EGF/Cr may be a reliable indicator of urinary EGF excretion in children with CRF .
	manualset3
125585	3	404494	13	NULL	NULL	0	NULL	glomerular filtration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results implicate that there is a functional relationship between glomerular filtration and urinary EGF excretion , and that the urinary EGF/Cr may be a reliable indicator of urinary EGF excretion in children with CRF .
	manualset3
125586	4	404494	13	NULL	NULL	0	NULL	urinary EGF excretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results implicate that there is a functional relationship between glomerular filtration and urinary EGF excretion , and that the urinary EGF/Cr may be a reliable indicator of urinary EGF excretion in children with CRF .
	manualset3
125587	5	404494	13	NULL	NULL	0	NULL	urinary EGF/Cr	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results implicate that there is a functional relationship between glomerular filtration and urinary EGF excretion , and that the urinary EGF/Cr may be a reliable indicator of urinary EGF excretion in children with CRF .
	manualset3
125603	6	404494	13	NULL	NULL	0	NULL	reliable indicator	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results implicate that there is a functional relationship between glomerular filtration and urinary EGF excretion , and that the urinary EGF/Cr may be a reliable indicator of urinary EGF excretion in children with CRF .
	manualset3
125604	7	404494	13	NULL	NULL	0	NULL	urinary EGF excretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results implicate that there is a functional relationship between glomerular filtration and urinary EGF excretion , and that the urinary EGF/Cr may be a reliable indicator of urinary EGF excretion in children with CRF .
	manualset3
125605	8	404494	13	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results implicate that there is a functional relationship between glomerular filtration and urinary EGF excretion , and that the urinary EGF/Cr may be a reliable indicator of urinary EGF excretion in children with CRF .
	manualset3
125606	9	404494	13	NULL	NULL	0	NULL	CRF	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results implicate that there is a functional relationship between glomerular filtration and urinary EGF excretion , and that the urinary EGF/Cr may be a reliable indicator of urinary EGF excretion in children with CRF .
	manualset3
125608	1	404495	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate extensive recombinatorial interactions between the homologous sequences at both loci leading to reconstitution of the cyanobacterial rbcL gene .
	manualset3
125609	2	404495	13	NULL	NULL	0	NULL	recombinatorial interactions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate extensive recombinatorial interactions between the homologous sequences at both loci leading to reconstitution of the cyanobacterial rbcL gene .
	manualset3
125610	3	404495	13	NULL	NULL	0	NULL	homologous sequences 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate extensive recombinatorial interactions between the homologous sequences at both loci leading to reconstitution of the cyanobacterial rbcL gene .
	manualset3
125611	4	404495	13	NULL	NULL	0	NULL	loci	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate extensive recombinatorial interactions between the homologous sequences at both loci leading to reconstitution of the cyanobacterial rbcL gene .
	manualset3
125613	5	404495	13	NULL	NULL	0	NULL	reconstitution 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate extensive recombinatorial interactions between the homologous sequences at both loci leading to reconstitution of the cyanobacterial rbcL gene .
	manualset3
125614	6	404495	13	NULL	NULL	0	NULL	cyanobacterial rbcL gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate extensive recombinatorial interactions between the homologous sequences at both loci leading to reconstitution of the cyanobacterial rbcL gene .
	manualset3
125938	1	404496	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that 15 ( S ) - HETE is an intracellular second messenger that facilitates translocation of PKCalpha to the membrane and elucidate a mechanism that plays a regulatory role in cell proliferation crucial to corneal wound healing .
	manualset3
125939	2	404496	13	NULL	NULL	0	NULL	15 ( S ) - HETE	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that 15 ( S ) - HETE is an intracellular second messenger that facilitates translocation of PKCalpha to the membrane and elucidate a mechanism that plays a regulatory role in cell proliferation crucial to corneal wound healing .
	manualset3
125940	3	404496	13	NULL	NULL	0	NULL	intracellular second messenger	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that 15 ( S ) - HETE is an intracellular second messenger that facilitates translocation of PKCalpha to the membrane and elucidate a mechanism that plays a regulatory role in cell proliferation crucial to corneal wound healing .
	manualset3
125941	4	404496	13	NULL	NULL	0	NULL	translocation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that 15 ( S ) - HETE is an intracellular second messenger that facilitates translocation of PKCalpha to the membrane and elucidate a mechanism that plays a regulatory role in cell proliferation crucial to corneal wound healing .
	manualset3
125942	5	404496	13	NULL	NULL	0	NULL	PKCalpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that 15 ( S ) - HETE is an intracellular second messenger that facilitates translocation of PKCalpha to the membrane and elucidate a mechanism that plays a regulatory role in cell proliferation crucial to corneal wound healing .
	manualset3
125943	6	404496	13	NULL	NULL	0	NULL	membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that 15 ( S ) - HETE is an intracellular second messenger that facilitates translocation of PKCalpha to the membrane and elucidate a mechanism that plays a regulatory role in cell proliferation crucial to corneal wound healing .
	manualset3
125944	7	404496	13	NULL	NULL	0	NULL	mechanism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that 15 ( S ) - HETE is an intracellular second messenger that facilitates translocation of PKCalpha to the membrane and elucidate a mechanism that plays a regulatory role in cell proliferation crucial to corneal wound healing .
	manualset3
125945	8	404496	13	NULL	NULL	0	NULL	regulatory role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that 15 ( S ) - HETE is an intracellular second messenger that facilitates translocation of PKCalpha to the membrane and elucidate a mechanism that plays a regulatory role in cell proliferation crucial to corneal wound healing .
	manualset3
125946	9	404496	13	NULL	NULL	0	NULL	cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that 15 ( S ) - HETE is an intracellular second messenger that facilitates translocation of PKCalpha to the membrane and elucidate a mechanism that plays a regulatory role in cell proliferation crucial to corneal wound healing .
	manualset3
125947	10	404496	13	NULL	NULL	0	NULL	corneal wound healing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that 15 ( S ) - HETE is an intracellular second messenger that facilitates translocation of PKCalpha to the membrane and elucidate a mechanism that plays a regulatory role in cell proliferation crucial to corneal wound healing .
	manualset3
125948	1	404497	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that 4-AP-induced seizures may be , at least in part , dependent on nitric oxide level .
	manualset3
125949	2	404497	13	NULL	NULL	0	NULL	4-AP-induced seizures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that 4-AP-induced seizures may be , at least in part , dependent on nitric oxide level .
	manualset3
125950	3	404497	13	NULL	NULL	0	NULL	nitric oxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that 4-AP-induced seizures may be , at least in part , dependent on nitric oxide level .
	manualset3
125951	4	404497	13	NULL	NULL	0	NULL	level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that 4-AP-induced seizures may be , at least in part , dependent on nitric oxide level .
	manualset3
125952	1	404498	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that OBP-401 causes viral spread into the regional lymphatic area and selectively replicates in neoplastic lesions , resulting in GFP expression in metastatic lymph nodes .
	manualset3
125953	2	404498	13	NULL	NULL	0	NULL	OBP-401	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that OBP-401 causes viral spread into the regional lymphatic area and selectively replicates in neoplastic lesions , resulting in GFP expression in metastatic lymph nodes .
	manualset3
125954	3	404498	13	NULL	NULL	0	NULL	regional lymphatic area	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that OBP-401 causes viral spread into the regional lymphatic area and selectively replicates in neoplastic lesions , resulting in GFP expression in metastatic lymph nodes .
	manualset3
125955	4	404498	13	NULL	NULL	0	NULL	replicates	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that OBP-401 causes viral spread into the regional lymphatic area and selectively replicates in neoplastic lesions , resulting in GFP expression in metastatic lymph nodes .
	manualset3
125956	5	404498	13	NULL	NULL	0	NULL	neoplastic lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that OBP-401 causes viral spread into the regional lymphatic area and selectively replicates in neoplastic lesions , resulting in GFP expression in metastatic lymph nodes .
	manualset3
125957	6	404498	13	NULL	NULL	0	NULL	GFP expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that OBP-401 causes viral spread into the regional lymphatic area and selectively replicates in neoplastic lesions , resulting in GFP expression in metastatic lymph nodes .
	manualset3
125958	7	404498	13	NULL	NULL	0	NULL	metastatic lymph nodes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that OBP-401 causes viral spread into the regional lymphatic area and selectively replicates in neoplastic lesions , resulting in GFP expression in metastatic lymph nodes .
	manualset3
125959	1	404499	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that T. cruzi upregulates GM-CSF release from MPM and from the two macrophage cell lines , activated ( or not ) by IFN-gamma .
	manualset3
125960	2	404499	13	NULL	NULL	0	NULL	T. cruzi 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that T. cruzi upregulates GM-CSF release from MPM and from the two macrophage cell lines , activated ( or not ) by IFN-gamma .
	manualset3
125961	3	404499	13	NULL	NULL	0	NULL	GM-CSF release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that T. cruzi upregulates GM-CSF release from MPM and from the two macrophage cell lines , activated ( or not ) by IFN-gamma .
	manualset3
125962	4	404499	13	NULL	NULL	0	NULL	MPM 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that T. cruzi upregulates GM-CSF release from MPM and from the two macrophage cell lines , activated ( or not ) by IFN-gamma .
	manualset3
125963	5	404499	13	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that T. cruzi upregulates GM-CSF release from MPM and from the two macrophage cell lines , activated ( or not ) by IFN-gamma .
	manualset3
125964	6	404499	13	NULL	NULL	0	NULL	macrophage cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that T. cruzi upregulates GM-CSF release from MPM and from the two macrophage cell lines , activated ( or not ) by IFN-gamma .
	manualset3
125965	7	404499	13	NULL	NULL	0	NULL	IFN-gamma	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that T. cruzi upregulates GM-CSF release from MPM and from the two macrophage cell lines , activated ( or not ) by IFN-gamma .
	manualset3
125966	1	404500	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that TGF-beta1 showed an intense intracellular marking pattern associated with fibroblasts , myofibroblasts , and capillary endothelial cells in all Dupuytren 's samples , regardless of disease stage .
	manualset3
125967	2	404500	13	NULL	NULL	0	NULL	TGF-beta1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that TGF-beta1 showed an intense intracellular marking pattern associated with fibroblasts , myofibroblasts , and capillary endothelial cells in all Dupuytren 's samples , regardless of disease stage .
	manualset3
125968	3	404500	13	NULL	NULL	0	NULL	 intracellular marking pattern	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that TGF-beta1 showed an intense intracellular marking pattern associated with fibroblasts , myofibroblasts , and capillary endothelial cells in all Dupuytren 's samples , regardless of disease stage .
	manualset3
125969	4	404500	13	NULL	NULL	0	NULL	fibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that TGF-beta1 showed an intense intracellular marking pattern associated with fibroblasts , myofibroblasts , and capillary endothelial cells in all Dupuytren 's samples , regardless of disease stage .
	manualset3
125970	5	404500	13	NULL	NULL	0	NULL	myofibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that TGF-beta1 showed an intense intracellular marking pattern associated with fibroblasts , myofibroblasts , and capillary endothelial cells in all Dupuytren 's samples , regardless of disease stage .
	manualset3
125971	6	404500	13	NULL	NULL	0	NULL	capillary endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that TGF-beta1 showed an intense intracellular marking pattern associated with fibroblasts , myofibroblasts , and capillary endothelial cells in all Dupuytren 's samples , regardless of disease stage .
	manualset3
125972	7	404500	13	NULL	NULL	0	NULL	Dupuytren 's samples	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that TGF-beta1 showed an intense intracellular marking pattern associated with fibroblasts , myofibroblasts , and capillary endothelial cells in all Dupuytren 's samples , regardless of disease stage .
	manualset3
125973	8	404500	13	NULL	NULL	0	NULL	disease stage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that TGF-beta1 showed an intense intracellular marking pattern associated with fibroblasts , myofibroblasts , and capillary endothelial cells in all Dupuytren 's samples , regardless of disease stage .
	manualset3
125974	1	404501	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that certain properties supporting perceptual grouping could be processed in the absence of awareness .
	manualset3
125975	2	404501	13	NULL	NULL	0	NULL	certain properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that certain properties supporting perceptual grouping could be processed in the absence of awareness .
	manualset3
125976	3	404501	13	NULL	NULL	0	NULL	perceptual grouping	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that certain properties supporting perceptual grouping could be processed in the absence of awareness .
	manualset3
125977	4	404501	13	NULL	NULL	0	NULL	absence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that certain properties supporting perceptual grouping could be processed in the absence of awareness .
	manualset3
125978	5	404501	13	NULL	NULL	0	NULL	awareness 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that certain properties supporting perceptual grouping could be processed in the absence of awareness .
	manualset3
125979	1	404502	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that the best conditions to obtain anti-snake antiserum from ammonium sulfate fractionated plasma are pH 3.3 , 3.5 g/l pepsin , digestion for 90 min at 37 degrees C , and 0.5 % caprylic acid .
	manualset3
125980	2	404502	13	NULL	NULL	0	NULL	best conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that the best conditions to obtain anti-snake antiserum from ammonium sulfate fractionated plasma are pH 3.3 , 3.5 g/l pepsin , digestion for 90 min at 37 degrees C , and 0.5 % caprylic acid .
	manualset3
125981	3	404502	13	NULL	NULL	0	NULL	anti-snake antiserum	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that the best conditions to obtain anti-snake antiserum from ammonium sulfate fractionated plasma are pH 3.3 , 3.5 g/l pepsin , digestion for 90 min at 37 degrees C , and 0.5 % caprylic acid .
	manualset3
125982	4	404502	13	NULL	NULL	0	NULL	ammonium sulfate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that the best conditions to obtain anti-snake antiserum from ammonium sulfate fractionated plasma are pH 3.3 , 3.5 g/l pepsin , digestion for 90 min at 37 degrees C , and 0.5 % caprylic acid .
	manualset3
125983	5	404502	13	NULL	NULL	0	NULL	plasma	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that the best conditions to obtain anti-snake antiserum from ammonium sulfate fractionated plasma are pH 3.3 , 3.5 g/l pepsin , digestion for 90 min at 37 degrees C , and 0.5 % caprylic acid .
	manualset3
125984	6	404502	13	NULL	NULL	0	NULL	pH 3.3	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that the best conditions to obtain anti-snake antiserum from ammonium sulfate fractionated plasma are pH 3.3 , 3.5 g/l pepsin , digestion for 90 min at 37 degrees C , and 0.5 % caprylic acid .
	manualset3
125985	7	404502	13	NULL	NULL	0	NULL	3.5 g/l 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that the best conditions to obtain anti-snake antiserum from ammonium sulfate fractionated plasma are pH 3.3 , 3.5 g/l pepsin , digestion for 90 min at 37 degrees C , and 0.5 % caprylic acid .
	manualset3
125986	8	404502	13	NULL	NULL	0	NULL	pepsin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that the best conditions to obtain anti-snake antiserum from ammonium sulfate fractionated plasma are pH 3.3 , 3.5 g/l pepsin , digestion for 90 min at 37 degrees C , and 0.5 % caprylic acid .
	manualset3
125987	9	404502	13	NULL	NULL	0	NULL	digestion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that the best conditions to obtain anti-snake antiserum from ammonium sulfate fractionated plasma are pH 3.3 , 3.5 g/l pepsin , digestion for 90 min at 37 degrees C , and 0.5 % caprylic acid .
	manualset3
125988	10	404502	13	NULL	NULL	0	NULL	90 min	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that the best conditions to obtain anti-snake antiserum from ammonium sulfate fractionated plasma are pH 3.3 , 3.5 g/l pepsin , digestion for 90 min at 37 degrees C , and 0.5 % caprylic acid .
	manualset3
125989	11	404502	13	NULL	NULL	0	NULL	37 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that the best conditions to obtain anti-snake antiserum from ammonium sulfate fractionated plasma are pH 3.3 , 3.5 g/l pepsin , digestion for 90 min at 37 degrees C , and 0.5 % caprylic acid .
	manualset3
125990	12	404502	13	NULL	NULL	0	NULL	0.5 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that the best conditions to obtain anti-snake antiserum from ammonium sulfate fractionated plasma are pH 3.3 , 3.5 g/l pepsin , digestion for 90 min at 37 degrees C , and 0.5 % caprylic acid .
	manualset3
125991	13	404502	13	NULL	NULL	0	NULL	caprylic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that the best conditions to obtain anti-snake antiserum from ammonium sulfate fractionated plasma are pH 3.3 , 3.5 g/l pepsin , digestion for 90 min at 37 degrees C , and 0.5 % caprylic acid .
	manualset3
125992	1	404503	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that wetland emissions dominated the inter-annual variability of methane sources , whereas fire emissions played a smaller role , except during the 1997-1998 El Nio event .
	manualset3
125993	2	404503	13	NULL	NULL	0	NULL	wetland	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that wetland emissions dominated the inter-annual variability of methane sources , whereas fire emissions played a smaller role , except during the 1997-1998 El Nio event .
	manualset3
125994	3	404503	13	NULL	NULL	0	NULL	emissions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that wetland emissions dominated the inter-annual variability of methane sources , whereas fire emissions played a smaller role , except during the 1997-1998 El Nio event .
	manualset3
125995	4	404503	13	NULL	NULL	0	NULL	variability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that wetland emissions dominated the inter-annual variability of methane sources , whereas fire emissions played a smaller role , except during the 1997-1998 El Nio event .
	manualset3
125996	5	404503	13	NULL	NULL	0	NULL	methane sources	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that wetland emissions dominated the inter-annual variability of methane sources , whereas fire emissions played a smaller role , except during the 1997-1998 El Nio event .
	manualset3
125997	6	404503	13	NULL	NULL	0	NULL	fire emissions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that wetland emissions dominated the inter-annual variability of methane sources , whereas fire emissions played a smaller role , except during the 1997-1998 El Nio event .
	manualset3
125998	7	404503	13	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that wetland emissions dominated the inter-annual variability of methane sources , whereas fire emissions played a smaller role , except during the 1997-1998 El Nio event .
	manualset3
125999	8	404503	13	NULL	NULL	0	NULL	1997-1998	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that wetland emissions dominated the inter-annual variability of methane sources , whereas fire emissions played a smaller role , except during the 1997-1998 El Nio event .
	manualset3
126000	9	404503	13	NULL	NULL	0	NULL	El Nio event	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that wetland emissions dominated the inter-annual variability of methane sources , whereas fire emissions played a smaller role , except during the 1997-1998 El Nio event .
	manualset3
126001	1	404504	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicated that AP-2 could significantly repress Mn-SOD promoter activity , and that this repression was both Mn-SOD promoter and AP-2-specific .
	manualset3
126002	2	404504	13	NULL	NULL	0	NULL	AP-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicated that AP-2 could significantly repress Mn-SOD promoter activity , and that this repression was both Mn-SOD promoter and AP-2-specific .
	manualset3
126003	3	404504	13	NULL	NULL	0	NULL	Mn-SOD promoter activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicated that AP-2 could significantly repress Mn-SOD promoter activity , and that this repression was both Mn-SOD promoter and AP-2-specific .
	manualset3
126004	4	404504	13	NULL	NULL	0	NULL	repression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicated that AP-2 could significantly repress Mn-SOD promoter activity , and that this repression was both Mn-SOD promoter and AP-2-specific .
	manualset3
126005	5	404504	13	NULL	NULL	0	NULL	Mn-SOD promoter 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicated that AP-2 could significantly repress Mn-SOD promoter activity , and that this repression was both Mn-SOD promoter and AP-2-specific .
	manualset3
126006	1	404505	13	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicated that yeast is a simple , effective alternative for NV VLP production .
	manualset3
126007	2	404505	13	NULL	NULL	0	NULL	yeast	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicated that yeast is a simple , effective alternative for NV VLP production .
	manualset3
126008	3	404505	13	NULL	NULL	0	NULL	alternative	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicated that yeast is a simple , effective alternative for NV VLP production .
	manualset3
126009	4	404505	13	NULL	NULL	0	NULL	NV VLP production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicated that yeast is a simple , effective alternative for NV VLP production .
	manualset3
126010	1	404506	13	NULL	NULL	0	NULL	duplex PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A duplex PCR to detect Bordetella pertussis and Bordetella parapertussis was developed with the insertion sequences IS481 ( B. pertussis ) and IS1001 ( B. parapertussis ) and evaluated with specimens from 520 consecutive patients presenting with possible pertussis .
	manualset3
126011	2	404506	13	NULL	NULL	0	NULL	Bordetella pertussis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A duplex PCR to detect Bordetella pertussis and Bordetella parapertussis was developed with the insertion sequences IS481 ( B. pertussis ) and IS1001 ( B. parapertussis ) and evaluated with specimens from 520 consecutive patients presenting with possible pertussis .
	manualset3
126012	3	404506	13	NULL	NULL	0	NULL	Bordetella parapertussis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A duplex PCR to detect Bordetella pertussis and Bordetella parapertussis was developed with the insertion sequences IS481 ( B. pertussis ) and IS1001 ( B. parapertussis ) and evaluated with specimens from 520 consecutive patients presenting with possible pertussis .
	manualset3
126013	4	404506	13	NULL	NULL	0	NULL	insertion sequences IS481 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A duplex PCR to detect Bordetella pertussis and Bordetella parapertussis was developed with the insertion sequences IS481 ( B. pertussis ) and IS1001 ( B. parapertussis ) and evaluated with specimens from 520 consecutive patients presenting with possible pertussis .
	manualset3
126014	5	404506	13	NULL	NULL	0	NULL	B. pertussis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A duplex PCR to detect Bordetella pertussis and Bordetella parapertussis was developed with the insertion sequences IS481 ( B. pertussis ) and IS1001 ( B. parapertussis ) and evaluated with specimens from 520 consecutive patients presenting with possible pertussis .
	manualset3
126015	6	404506	13	NULL	NULL	0	NULL	insertion sequences IS1001	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A duplex PCR to detect Bordetella pertussis and Bordetella parapertussis was developed with the insertion sequences IS481 ( B. pertussis ) and IS1001 ( B. parapertussis ) and evaluated with specimens from 520 consecutive patients presenting with possible pertussis .
	manualset3
126016	7	404506	13	NULL	NULL	0	NULL	B. parapertussis 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A duplex PCR to detect Bordetella pertussis and Bordetella parapertussis was developed with the insertion sequences IS481 ( B. pertussis ) and IS1001 ( B. parapertussis ) and evaluated with specimens from 520 consecutive patients presenting with possible pertussis .
	manualset3
126017	8	404506	13	NULL	NULL	0	NULL	specimens	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A duplex PCR to detect Bordetella pertussis and Bordetella parapertussis was developed with the insertion sequences IS481 ( B. pertussis ) and IS1001 ( B. parapertussis ) and evaluated with specimens from 520 consecutive patients presenting with possible pertussis .
	manualset3
126018	9	404506	13	NULL	NULL	0	NULL	520 consecutive patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A duplex PCR to detect Bordetella pertussis and Bordetella parapertussis was developed with the insertion sequences IS481 ( B. pertussis ) and IS1001 ( B. parapertussis ) and evaluated with specimens from 520 consecutive patients presenting with possible pertussis .
	manualset3
126019	10	404506	13	NULL	NULL	0	NULL	pertussis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A duplex PCR to detect Bordetella pertussis and Bordetella parapertussis was developed with the insertion sequences IS481 ( B. pertussis ) and IS1001 ( B. parapertussis ) and evaluated with specimens from 520 consecutive patients presenting with possible pertussis .
	manualset3
126020	1	404507	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results provide evidence for a link between GLUT12 protein trafficking , glucose transport and signaling molecules central to the control of metabolic disease processes .
	manualset3
126021	2	404507	13	NULL	NULL	0	NULL	evidence 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results provide evidence for a link between GLUT12 protein trafficking , glucose transport and signaling molecules central to the control of metabolic disease processes .
	manualset3
126022	3	404507	13	NULL	NULL	0	NULL	link	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results provide evidence for a link between GLUT12 protein trafficking , glucose transport and signaling molecules central to the control of metabolic disease processes .
	manualset3
126023	4	404507	13	NULL	NULL	0	NULL	GLUT12 protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results provide evidence for a link between GLUT12 protein trafficking , glucose transport and signaling molecules central to the control of metabolic disease processes .
	manualset3
126024	5	404507	13	NULL	NULL	0	NULL	glucose transport	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results provide evidence for a link between GLUT12 protein trafficking , glucose transport and signaling molecules central to the control of metabolic disease processes .
	manualset3
126025	6	404507	13	NULL	NULL	0	NULL	signaling molecules	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results provide evidence for a link between GLUT12 protein trafficking , glucose transport and signaling molecules central to the control of metabolic disease processes .
	manualset3
126026	7	404507	13	NULL	NULL	0	NULL	control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results provide evidence for a link between GLUT12 protein trafficking , glucose transport and signaling molecules central to the control of metabolic disease processes .
	manualset3
126027	8	404507	13	NULL	NULL	0	NULL	metabolic disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results provide evidence for a link between GLUT12 protein trafficking , glucose transport and signaling molecules central to the control of metabolic disease processes .
	manualset3
126028	9	404507	13	NULL	NULL	0	NULL	processes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results provide evidence for a link between GLUT12 protein trafficking , glucose transport and signaling molecules central to the control of metabolic disease processes .
	manualset3
126029	1	404508	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results provide evidence that developmental nicotine exposure is responsible for auditory-cognitive deficits in the offspring of women who smoke during pregnancy , and suggest a potential underlying mechanism , namely diminished function of cortical nAChRs .
	manualset3
126030	2	404508	13	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results provide evidence that developmental nicotine exposure is responsible for auditory-cognitive deficits in the offspring of women who smoke during pregnancy , and suggest a potential underlying mechanism , namely diminished function of cortical nAChRs .
	manualset3
126031	3	404508	13	NULL	NULL	0	NULL	nicotine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results provide evidence that developmental nicotine exposure is responsible for auditory-cognitive deficits in the offspring of women who smoke during pregnancy , and suggest a potential underlying mechanism , namely diminished function of cortical nAChRs .
	manualset3
126032	4	404508	13	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results provide evidence that developmental nicotine exposure is responsible for auditory-cognitive deficits in the offspring of women who smoke during pregnancy , and suggest a potential underlying mechanism , namely diminished function of cortical nAChRs .
	manualset3
126033	5	404508	13	NULL	NULL	0	NULL	auditory-cognitive deficits 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results provide evidence that developmental nicotine exposure is responsible for auditory-cognitive deficits in the offspring of women who smoke during pregnancy , and suggest a potential underlying mechanism , namely diminished function of cortical nAChRs .
	manualset3
126034	6	404508	13	NULL	NULL	0	NULL	offspring 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results provide evidence that developmental nicotine exposure is responsible for auditory-cognitive deficits in the offspring of women who smoke during pregnancy , and suggest a potential underlying mechanism , namely diminished function of cortical nAChRs .
	manualset3
126035	7	404508	13	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results provide evidence that developmental nicotine exposure is responsible for auditory-cognitive deficits in the offspring of women who smoke during pregnancy , and suggest a potential underlying mechanism , namely diminished function of cortical nAChRs .
	manualset3
126037	9	404508	13	NULL	NULL	0	NULL	pregnancy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results provide evidence that developmental nicotine exposure is responsible for auditory-cognitive deficits in the offspring of women who smoke during pregnancy , and suggest a potential underlying mechanism , namely diminished function of cortical nAChRs .
	manualset3
126038	10	404508	13	NULL	NULL	0	NULL	mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results provide evidence that developmental nicotine exposure is responsible for auditory-cognitive deficits in the offspring of women who smoke during pregnancy , and suggest a potential underlying mechanism , namely diminished function of cortical nAChRs .
	manualset3
126039	11	404508	13	NULL	NULL	NULL	NULL	function	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our results provide evidence that developmental nicotine exposure is responsible for auditory-cognitive deficits in the offspring of women who smoke during pregnancy , and suggest a potential underlying mechanism , namely diminished function of cortical nAChRs .
	manualset3
126040	12	404508	13	NULL	NULL	0	NULL	cortical nAChRs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results provide evidence that developmental nicotine exposure is responsible for auditory-cognitive deficits in the offspring of women who smoke during pregnancy , and suggest a potential underlying mechanism , namely diminished function of cortical nAChRs .
	manualset3
126041	1	404509	13	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results provide the morphological basis for further studies of the function of the labeled neurons and new insights into NO/cGMP signalling .
	manualset3
126042	2	404509	13	NULL	NULL	0	NULL	morphological basis	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results provide the morphological basis for further studies of the function of the labeled neurons and new insights into NO/cGMP signalling .
	manualset3
126043	3	404509	13	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results provide the morphological basis for further studies of the function of the labeled neurons and new insights into NO/cGMP signalling .
	manualset3
126044	4	404509	13	NULL	NULL	0	NULL	function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results provide the morphological basis for further studies of the function of the labeled neurons and new insights into NO/cGMP signalling .
	manualset3
126045	5	404509	13	NULL	NULL	0	NULL	neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results provide the morphological basis for further studies of the function of the labeled neurons and new insights into NO/cGMP signalling .
	manualset3
126046	6	404509	13	NULL	NULL	0	NULL	insights	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results provide the morphological basis for further studies of the function of the labeled neurons and new insights into NO/cGMP signalling .
	manualset3
126047	7	404509	13	NULL	NULL	0	NULL	NO/cGMP signalling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results provide the morphological basis for further studies of the function of the labeled neurons and new insights into NO/cGMP signalling .
	manualset3
126048	1	404510	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results render further evidence that LGTMRN is a distinct entity from the hitherto established renal neoplasms .
	manualset3
126049	2	404510	13	NULL	NULL	0	NULL	evidence 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results render further evidence that LGTMRN is a distinct entity from the hitherto established renal neoplasms .
	manualset3
126050	3	404510	13	NULL	NULL	0	NULL	LGTMRN	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results render further evidence that LGTMRN is a distinct entity from the hitherto established renal neoplasms .
	manualset3
126051	4	404510	13	NULL	NULL	0	NULL	distinct entity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results render further evidence that LGTMRN is a distinct entity from the hitherto established renal neoplasms .
	manualset3
126052	5	404510	13	NULL	NULL	0	NULL	renal neoplasms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results render further evidence that LGTMRN is a distinct entity from the hitherto established renal neoplasms .
	manualset3
126053	1	404511	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results reveal a novel mechanism by which AMPK regulates ER homeostasis in hepatocytes and suggest that AMPK has a protective role against hypercholesterolemia-related liver damage .
	manualset3
126054	2	404511	13	NULL	NULL	0	NULL	mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results reveal a novel mechanism by which AMPK regulates ER homeostasis in hepatocytes and suggest that AMPK has a protective role against hypercholesterolemia-related liver damage .
	manualset3
126055	3	404511	13	NULL	NULL	0	NULL	AMPK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results reveal a novel mechanism by which AMPK regulates ER homeostasis in hepatocytes and suggest that AMPK has a protective role against hypercholesterolemia-related liver damage .
	manualset3
126056	4	404511	13	NULL	NULL	0	NULL	ER homeostasis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results reveal a novel mechanism by which AMPK regulates ER homeostasis in hepatocytes and suggest that AMPK has a protective role against hypercholesterolemia-related liver damage .
	manualset3
126057	5	404511	13	NULL	NULL	0	NULL	hepatocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results reveal a novel mechanism by which AMPK regulates ER homeostasis in hepatocytes and suggest that AMPK has a protective role against hypercholesterolemia-related liver damage .
	manualset3
126058	6	404511	13	NULL	NULL	0	NULL	AMPK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results reveal a novel mechanism by which AMPK regulates ER homeostasis in hepatocytes and suggest that AMPK has a protective role against hypercholesterolemia-related liver damage .
	manualset3
126059	7	404511	13	NULL	NULL	0	NULL	protective role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results reveal a novel mechanism by which AMPK regulates ER homeostasis in hepatocytes and suggest that AMPK has a protective role against hypercholesterolemia-related liver damage .
	manualset3
126060	8	404511	13	NULL	NULL	0	NULL	hypercholesterolemia-related liver damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results reveal a novel mechanism by which AMPK regulates ER homeostasis in hepatocytes and suggest that AMPK has a protective role against hypercholesterolemia-related liver damage .
	manualset3
126061	1	404512	13	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results revealed that bee venom pretreatment ( 1-100ng / ml ) increased the cell viability and decreased apoptosis assessed by DNA fragmentation and caspase-3 activity assays in MPP ( + ) - induced cytotoxicity in SH-SY5Y cells .
	manualset3
126062	2	404512	13	NULL	NULL	0	NULL	venom	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results revealed that bee venom pretreatment ( 1-100ng / ml ) increased the cell viability and decreased apoptosis assessed by DNA fragmentation and caspase-3 activity assays in MPP ( + ) - induced cytotoxicity in SH-SY5Y cells .
	manualset3
126063	3	404512	13	NULL	NULL	0	NULL	pretreatment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results revealed that bee venom pretreatment ( 1-100ng / ml ) increased the cell viability and decreased apoptosis assessed by DNA fragmentation and caspase-3 activity assays in MPP ( + ) - induced cytotoxicity in SH-SY5Y cells .
	manualset3
126064	4	404512	13	NULL	NULL	0	NULL	1-100ng / ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results revealed that bee venom pretreatment ( 1-100ng / ml ) increased the cell viability and decreased apoptosis assessed by DNA fragmentation and caspase-3 activity assays in MPP ( + ) - induced cytotoxicity in SH-SY5Y cells .
	manualset3
126065	5	404512	13	NULL	NULL	0	NULL	cell viability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results revealed that bee venom pretreatment ( 1-100ng / ml ) increased the cell viability and decreased apoptosis assessed by DNA fragmentation and caspase-3 activity assays in MPP ( + ) - induced cytotoxicity in SH-SY5Y cells .
	manualset3
126066	6	404512	13	NULL	NULL	0	NULL	apoptosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results revealed that bee venom pretreatment ( 1-100ng / ml ) increased the cell viability and decreased apoptosis assessed by DNA fragmentation and caspase-3 activity assays in MPP ( + ) - induced cytotoxicity in SH-SY5Y cells .
	manualset3
126067	7	404512	13	NULL	NULL	NULL	NULL	DNA fragmentation assays	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our results revealed that bee venom pretreatment ( 1-100ng / ml ) increased the cell viability and decreased apoptosis assessed by DNA fragmentation and caspase-3 activity assays in MPP ( + ) - induced cytotoxicity in SH-SY5Y cells .
	manualset3
126068	8	404512	13	NULL	NULL	0	NULL	caspase-3 activity assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results revealed that bee venom pretreatment ( 1-100ng / ml ) increased the cell viability and decreased apoptosis assessed by DNA fragmentation and caspase-3 activity assays in MPP ( + ) - induced cytotoxicity in SH-SY5Y cells .
	manualset3
126069	9	404512	13	NULL	NULL	0	NULL	MPP ( + ) - induced cytotoxicity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results revealed that bee venom pretreatment ( 1-100ng / ml ) increased the cell viability and decreased apoptosis assessed by DNA fragmentation and caspase-3 activity assays in MPP ( + ) - induced cytotoxicity in SH-SY5Y cells .
	manualset3
126070	10	404512	13	NULL	NULL	0	NULL	SH-SY5Y cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results revealed that bee venom pretreatment ( 1-100ng / ml ) increased the cell viability and decreased apoptosis assessed by DNA fragmentation and caspase-3 activity assays in MPP ( + ) - induced cytotoxicity in SH-SY5Y cells .
	manualset3
126071	1	404513	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results revealed that morphine induced a robust CPP in wild-type mice but not in mice lacking the opioid receptor or in wild-type mice treated with - FNA .
	manualset3
126072	2	404513	13	NULL	NULL	0	NULL	morphine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results revealed that morphine induced a robust CPP in wild-type mice but not in mice lacking the opioid receptor or in wild-type mice treated with - FNA .
	manualset3
126073	3	404513	13	NULL	NULL	0	NULL	robust CPP	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results revealed that morphine induced a robust CPP in wild-type mice but not in mice lacking the opioid receptor or in wild-type mice treated with - FNA .
	manualset3
126074	4	404513	13	NULL	NULL	0	NULL	wild-type mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results revealed that morphine induced a robust CPP in wild-type mice but not in mice lacking the opioid receptor or in wild-type mice treated with - FNA .
	manualset3
126075	5	404513	13	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results revealed that morphine induced a robust CPP in wild-type mice but not in mice lacking the opioid receptor or in wild-type mice treated with - FNA .
	manualset3
126076	6	404513	13	NULL	NULL	0	NULL	opioid receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results revealed that morphine induced a robust CPP in wild-type mice but not in mice lacking the opioid receptor or in wild-type mice treated with - FNA .
	manualset3
126077	7	404513	13	NULL	NULL	0	NULL	wild-type mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results revealed that morphine induced a robust CPP in wild-type mice but not in mice lacking the opioid receptor or in wild-type mice treated with - FNA .
	manualset3
126078	8	404513	13	NULL	NULL	0	NULL	FNA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results revealed that morphine induced a robust CPP in wild-type mice but not in mice lacking the opioid receptor or in wild-type mice treated with - FNA .
	manualset3
126079	1	404514	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results revealed that this antibody also catalyzed the redox reaction of resazurin to resorufin , which are both structurally related to fluorescein .
	manualset3
126080	2	404514	13	NULL	NULL	0	NULL	antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results revealed that this antibody also catalyzed the redox reaction of resazurin to resorufin , which are both structurally related to fluorescein .
	manualset3
126081	3	404514	13	NULL	NULL	0	NULL	redox reaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results revealed that this antibody also catalyzed the redox reaction of resazurin to resorufin , which are both structurally related to fluorescein .
	manualset3
126082	4	404514	13	NULL	NULL	0	NULL	resazurin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results revealed that this antibody also catalyzed the redox reaction of resazurin to resorufin , which are both structurally related to fluorescein .
	manualset3
126083	5	404514	13	NULL	NULL	0	NULL	resorufin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results revealed that this antibody also catalyzed the redox reaction of resazurin to resorufin , which are both structurally related to fluorescein .
	manualset3
126084	6	404514	13	NULL	NULL	0	NULL	fluorescein	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results revealed that this antibody also catalyzed the redox reaction of resazurin to resorufin , which are both structurally related to fluorescein .
	manualset3
126085	1	404515	13	NULL	NULL	0	NULL	dust dispenser	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A dust dispenser for deliquescent-material .
	manualset3
126086	1	404516	13	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that HR rats exhibited a decrease in thymus weight after repeated social defeat that was not present in LRs .
	manualset3
126087	2	404516	13	NULL	NULL	0	NULL	HR rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that HR rats exhibited a decrease in thymus weight after repeated social defeat that was not present in LRs .
	manualset3
126088	3	404516	13	NULL	NULL	0	NULL	decrease 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that HR rats exhibited a decrease in thymus weight after repeated social defeat that was not present in LRs .
	manualset3
126089	4	404516	13	NULL	NULL	0	NULL	thymus weight	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that HR rats exhibited a decrease in thymus weight after repeated social defeat that was not present in LRs .
	manualset3
126090	5	404516	13	NULL	NULL	0	NULL	social defeat	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that HR rats exhibited a decrease in thymus weight after repeated social defeat that was not present in LRs .
	manualset3
126091	6	404516	13	NULL	NULL	0	NULL	LRs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that HR rats exhibited a decrease in thymus weight after repeated social defeat that was not present in LRs .
	manualset3
126092	1	404517	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that RA treatment causes a strong enhancement in c-jun promoter activity , an effect probably mediated by the RA-receptor beta ( RAR beta ) .
	manualset3
126093	2	404517	13	NULL	NULL	0	NULL	RA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that RA treatment causes a strong enhancement in c-jun promoter activity , an effect probably mediated by the RA-receptor beta ( RAR beta ) .
	manualset3
126094	3	404517	13	NULL	NULL	0	NULL	treatment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that RA treatment causes a strong enhancement in c-jun promoter activity , an effect probably mediated by the RA-receptor beta ( RAR beta ) .
	manualset3
126095	4	404517	13	NULL	NULL	0	NULL	enhancement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that RA treatment causes a strong enhancement in c-jun promoter activity , an effect probably mediated by the RA-receptor beta ( RAR beta ) .
	manualset3
126096	5	404517	13	NULL	NULL	0	NULL	c-jun promoter activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that RA treatment causes a strong enhancement in c-jun promoter activity , an effect probably mediated by the RA-receptor beta ( RAR beta ) .
	manualset3
126097	6	404517	13	NULL	NULL	0	NULL	effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that RA treatment causes a strong enhancement in c-jun promoter activity , an effect probably mediated by the RA-receptor beta ( RAR beta ) .
	manualset3
126098	7	404517	13	NULL	NULL	0	NULL	RA-receptor beta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that RA treatment causes a strong enhancement in c-jun promoter activity , an effect probably mediated by the RA-receptor beta ( RAR beta ) .
	manualset3
126099	8	404517	13	NULL	NULL	0	NULL	RAR beta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that RA treatment causes a strong enhancement in c-jun promoter activity , an effect probably mediated by the RA-receptor beta ( RAR beta ) .
	manualset3
126107	1	404518	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that genes that respond early at the site of the wound also respond throughout the plant , with similar kinetics .
	manualset3
126108	2	404518	13	NULL	NULL	0	NULL	genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that genes that respond early at the site of the wound also respond throughout the plant , with similar kinetics .
	manualset3
126112	3	404518	13	NULL	NULL	0	NULL	site	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that genes that respond early at the site of the wound also respond throughout the plant , with similar kinetics .
	manualset3
126113	4	404518	13	NULL	NULL	0	NULL	wound	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that genes that respond early at the site of the wound also respond throughout the plant , with similar kinetics .
	manualset3
126115	5	404518	13	NULL	NULL	0	NULL	plant	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that genes that respond early at the site of the wound also respond throughout the plant , with similar kinetics .
	manualset3
126116	6	404518	13	NULL	NULL	0	NULL	kinetics 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that genes that respond early at the site of the wound also respond throughout the plant , with similar kinetics .
	manualset3
126118	1	404519	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that in patients with stable asthma , there is an increased plasma exudation into the airways , most likely caused by an increased respiratory membrane permeability .
	manualset3
126120	2	404519	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that in patients with stable asthma , there is an increased plasma exudation into the airways , most likely caused by an increased respiratory membrane permeability .
	manualset3
126121	3	404519	13	NULL	NULL	0	NULL	asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that in patients with stable asthma , there is an increased plasma exudation into the airways , most likely caused by an increased respiratory membrane permeability .
	manualset3
126122	4	404519	13	NULL	NULL	0	NULL	plasma exudation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that in patients with stable asthma , there is an increased plasma exudation into the airways , most likely caused by an increased respiratory membrane permeability .
	manualset3
126123	5	404519	13	NULL	NULL	0	NULL	airways	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that in patients with stable asthma , there is an increased plasma exudation into the airways , most likely caused by an increased respiratory membrane permeability .
	manualset3
126125	6	404519	13	NULL	NULL	0	NULL	respiratory membrane 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that in patients with stable asthma , there is an increased plasma exudation into the airways , most likely caused by an increased respiratory membrane permeability .
	manualset3
126126	7	404519	13	NULL	NULL	0	NULL	permeability 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that in patients with stable asthma , there is an increased plasma exudation into the airways , most likely caused by an increased respiratory membrane permeability .
	manualset3
126130	1	404520	13	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that the cell adhesion molecule contactin binds directly to Na ( v ) 1.9 / NaN and recruits tenascin to the protein complex in vitro .
	manualset3
126132	2	404520	13	NULL	NULL	0	NULL	cell adhesion molecule	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that the cell adhesion molecule contactin binds directly to Na ( v ) 1.9 / NaN and recruits tenascin to the protein complex in vitro .
	manualset3
126133	3	404520	13	NULL	NULL	0	NULL	contactin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that the cell adhesion molecule contactin binds directly to Na ( v ) 1.9 / NaN and recruits tenascin to the protein complex in vitro .
	manualset3
126137	4	404520	13	NULL	NULL	0	NULL	Na ( v ) 1.9 / NaN 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that the cell adhesion molecule contactin binds directly to Na ( v ) 1.9 / NaN and recruits tenascin to the protein complex in vitro .
	manualset3
126139	5	404520	13	NULL	NULL	0	NULL	recruits 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that the cell adhesion molecule contactin binds directly to Na ( v ) 1.9 / NaN and recruits tenascin to the protein complex in vitro .
	manualset3
126141	6	404520	13	NULL	NULL	0	NULL	tenascin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that the cell adhesion molecule contactin binds directly to Na ( v ) 1.9 / NaN and recruits tenascin to the protein complex in vitro .
	manualset3
126142	7	404520	13	NULL	NULL	0	NULL	protein complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that the cell adhesion molecule contactin binds directly to Na ( v ) 1.9 / NaN and recruits tenascin to the protein complex in vitro .
	manualset3
126168	1	404521	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that the fraction of patients with high-grade tumors that fall outside trials designed for ` classical osteosarcoma ' may be larger than is usually acknowledged , and that the results reported for the classical group are by no means representative of the whole patient population .
	manualset3
126169	2	404521	13	NULL	NULL	0	NULL	fraction	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that the fraction of patients with high-grade tumors that fall outside trials designed for ` classical osteosarcoma ' may be larger than is usually acknowledged , and that the results reported for the classical group are by no means representative of the whole patient population .
	manualset3
126170	3	404521	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that the fraction of patients with high-grade tumors that fall outside trials designed for ` classical osteosarcoma ' may be larger than is usually acknowledged , and that the results reported for the classical group are by no means representative of the whole patient population .
	manualset3
126171	4	404521	13	NULL	NULL	0	NULL	high-grade tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that the fraction of patients with high-grade tumors that fall outside trials designed for ` classical osteosarcoma ' may be larger than is usually acknowledged , and that the results reported for the classical group are by no means representative of the whole patient population .
	manualset3
126172	5	404521	13	NULL	NULL	0	NULL	trials	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that the fraction of patients with high-grade tumors that fall outside trials designed for ` classical osteosarcoma ' may be larger than is usually acknowledged , and that the results reported for the classical group are by no means representative of the whole patient population .
	manualset3
126173	6	404521	13	NULL	NULL	0	NULL	classical osteosarcoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that the fraction of patients with high-grade tumors that fall outside trials designed for ` classical osteosarcoma ' may be larger than is usually acknowledged , and that the results reported for the classical group are by no means representative of the whole patient population .
	manualset3
126174	7	404521	13	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that the fraction of patients with high-grade tumors that fall outside trials designed for ` classical osteosarcoma ' may be larger than is usually acknowledged , and that the results reported for the classical group are by no means representative of the whole patient population .
	manualset3
126175	8	404521	13	NULL	NULL	0	NULL	classical group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that the fraction of patients with high-grade tumors that fall outside trials designed for ` classical osteosarcoma ' may be larger than is usually acknowledged , and that the results reported for the classical group are by no means representative of the whole patient population .
	manualset3
126176	9	404521	13	NULL	NULL	0	NULL	patient population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that the fraction of patients with high-grade tumors that fall outside trials designed for ` classical osteosarcoma ' may be larger than is usually acknowledged , and that the results reported for the classical group are by no means representative of the whole patient population .
	manualset3
126177	1	404522	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed how chemoreceptors directed bacterial chemotaxis within cylindroids : the aspartate receptor initiated chemotaxis toward cylindroids , the serine receptor initiated penetration , and the ribose/galactose receptor directed S. typhimurium toward necrosis .
	manualset3
126178	2	404522	13	NULL	NULL	0	NULL	chemoreceptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed how chemoreceptors directed bacterial chemotaxis within cylindroids : the aspartate receptor initiated chemotaxis toward cylindroids , the serine receptor initiated penetration , and the ribose/galactose receptor directed S. typhimurium toward necrosis .
	manualset3
126179	3	404522	13	NULL	NULL	0	NULL	bacterial chemotaxis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed how chemoreceptors directed bacterial chemotaxis within cylindroids : the aspartate receptor initiated chemotaxis toward cylindroids , the serine receptor initiated penetration , and the ribose/galactose receptor directed S. typhimurium toward necrosis .
	manualset3
126180	4	404522	13	NULL	NULL	0	NULL	cylindroids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed how chemoreceptors directed bacterial chemotaxis within cylindroids : the aspartate receptor initiated chemotaxis toward cylindroids , the serine receptor initiated penetration , and the ribose/galactose receptor directed S. typhimurium toward necrosis .
	manualset3
126181	5	404522	13	NULL	NULL	0	NULL	aspartate receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed how chemoreceptors directed bacterial chemotaxis within cylindroids : the aspartate receptor initiated chemotaxis toward cylindroids , the serine receptor initiated penetration , and the ribose/galactose receptor directed S. typhimurium toward necrosis .
	manualset3
126182	6	404522	13	NULL	NULL	0	NULL	chemotaxis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed how chemoreceptors directed bacterial chemotaxis within cylindroids : the aspartate receptor initiated chemotaxis toward cylindroids , the serine receptor initiated penetration , and the ribose/galactose receptor directed S. typhimurium toward necrosis .
	manualset3
126183	7	404522	13	NULL	NULL	0	NULL	cylindroids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed how chemoreceptors directed bacterial chemotaxis within cylindroids : the aspartate receptor initiated chemotaxis toward cylindroids , the serine receptor initiated penetration , and the ribose/galactose receptor directed S. typhimurium toward necrosis .
	manualset3
126184	8	404522	13	NULL	NULL	0	NULL	serine receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed how chemoreceptors directed bacterial chemotaxis within cylindroids : the aspartate receptor initiated chemotaxis toward cylindroids , the serine receptor initiated penetration , and the ribose/galactose receptor directed S. typhimurium toward necrosis .
	manualset3
126185	9	404522	13	NULL	NULL	0	NULL	penetration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed how chemoreceptors directed bacterial chemotaxis within cylindroids : the aspartate receptor initiated chemotaxis toward cylindroids , the serine receptor initiated penetration , and the ribose/galactose receptor directed S. typhimurium toward necrosis .
	manualset3
126186	10	404522	13	NULL	NULL	0	NULL	ribose/galactose receptor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed how chemoreceptors directed bacterial chemotaxis within cylindroids : the aspartate receptor initiated chemotaxis toward cylindroids , the serine receptor initiated penetration , and the ribose/galactose receptor directed S. typhimurium toward necrosis .
	manualset3
126187	11	404522	13	NULL	NULL	0	NULL	S. typhimurium	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed how chemoreceptors directed bacterial chemotaxis within cylindroids : the aspartate receptor initiated chemotaxis toward cylindroids , the serine receptor initiated penetration , and the ribose/galactose receptor directed S. typhimurium toward necrosis .
	manualset3
126188	12	404522	13	NULL	NULL	0	NULL	necrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed how chemoreceptors directed bacterial chemotaxis within cylindroids : the aspartate receptor initiated chemotaxis toward cylindroids , the serine receptor initiated penetration , and the ribose/galactose receptor directed S. typhimurium toward necrosis .
	manualset3
126189	1	404523	13	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that Erk1/2 played an important role in the interplay between cell-extrinsic cues and cell-intrinsic genetic mechanisms in neural stem cell biology .
	manualset3
126190	2	404523	13	NULL	NULL	0	NULL	Erk1/2 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that Erk1/2 played an important role in the interplay between cell-extrinsic cues and cell-intrinsic genetic mechanisms in neural stem cell biology .
	manualset3
126191	3	404523	13	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that Erk1/2 played an important role in the interplay between cell-extrinsic cues and cell-intrinsic genetic mechanisms in neural stem cell biology .
	manualset3
126192	4	404523	13	NULL	NULL	0	NULL	cell-extrinsic cues	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that Erk1/2 played an important role in the interplay between cell-extrinsic cues and cell-intrinsic genetic mechanisms in neural stem cell biology .
	manualset3
126193	5	404523	13	NULL	NULL	0	NULL	cell-intrinsic genetic mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that Erk1/2 played an important role in the interplay between cell-extrinsic cues and cell-intrinsic genetic mechanisms in neural stem cell biology .
	manualset3
126194	6	404523	13	NULL	NULL	0	NULL	neural stem cell biology 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that Erk1/2 played an important role in the interplay between cell-extrinsic cues and cell-intrinsic genetic mechanisms in neural stem cell biology .
	manualset3
126195	1	404524	13	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that fully differentiated cells from hMSCs were capable of dedifferentiation and transdifferentiation into cells of another developmental lineage at single cell levels .
	manualset3
126196	2	404524	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that fully differentiated cells from hMSCs were capable of dedifferentiation and transdifferentiation into cells of another developmental lineage at single cell levels .
	manualset3
126197	3	404524	13	NULL	NULL	0	NULL	hMSCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that fully differentiated cells from hMSCs were capable of dedifferentiation and transdifferentiation into cells of another developmental lineage at single cell levels .
	manualset3
126198	4	404524	13	NULL	NULL	0	NULL	dedifferentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that fully differentiated cells from hMSCs were capable of dedifferentiation and transdifferentiation into cells of another developmental lineage at single cell levels .
	manualset3
126199	5	404524	13	NULL	NULL	0	NULL	transdifferentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that fully differentiated cells from hMSCs were capable of dedifferentiation and transdifferentiation into cells of another developmental lineage at single cell levels .
	manualset3
126200	6	404524	13	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that fully differentiated cells from hMSCs were capable of dedifferentiation and transdifferentiation into cells of another developmental lineage at single cell levels .
	manualset3
126201	7	404524	13	NULL	NULL	0	NULL	developmental lineage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that fully differentiated cells from hMSCs were capable of dedifferentiation and transdifferentiation into cells of another developmental lineage at single cell levels .
	manualset3
126202	8	404524	13	NULL	NULL	0	NULL	single cell levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that fully differentiated cells from hMSCs were capable of dedifferentiation and transdifferentiation into cells of another developmental lineage at single cell levels .
	manualset3
126203	1	404525	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that it preferred to bind with G-quadruplex in c-myc and had rather insignificant effect on G-quadruplex in telomere .
	manualset3
126204	2	404525	13	NULL	NULL	0	NULL	G-quadruplex	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that it preferred to bind with G-quadruplex in c-myc and had rather insignificant effect on G-quadruplex in telomere .
	manualset3
126205	3	404525	13	NULL	NULL	0	NULL	c-myc	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that it preferred to bind with G-quadruplex in c-myc and had rather insignificant effect on G-quadruplex in telomere .
	manualset3
126206	4	404525	13	NULL	NULL	0	NULL	effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that it preferred to bind with G-quadruplex in c-myc and had rather insignificant effect on G-quadruplex in telomere .
	manualset3
126207	5	404525	13	NULL	NULL	0	NULL	G-quadruplex	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that it preferred to bind with G-quadruplex in c-myc and had rather insignificant effect on G-quadruplex in telomere .
	manualset3
126208	6	404525	13	NULL	NULL	NULL	NULL	telomere	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our results showed that it preferred to bind with G-quadruplex in c-myc and had rather insignificant effect on G-quadruplex in telomere .
	manualset3
126209	1	404526	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that microtubule interfering agents , paclitaxel ( 1-5 microM ) , colchicine ( 1-100 microM ) , nocodazole ( 1-20 microM ) , and vincristine ( 1-50 microM ) , did not affect either PMA or fMLP-induced oxidative burst .
	manualset3
126210	2	404526	13	NULL	NULL	0	NULL	microtubule interfering agents	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that microtubule interfering agents , paclitaxel ( 1-5 microM ) , colchicine ( 1-100 microM ) , nocodazole ( 1-20 microM ) , and vincristine ( 1-50 microM ) , did not affect either PMA or fMLP-induced oxidative burst .
	manualset3
126211	3	404526	13	NULL	NULL	0	NULL	paclitaxel	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that microtubule interfering agents , paclitaxel ( 1-5 microM ) , colchicine ( 1-100 microM ) , nocodazole ( 1-20 microM ) , and vincristine ( 1-50 microM ) , did not affect either PMA or fMLP-induced oxidative burst .
	manualset3
126212	4	404526	13	NULL	NULL	0	NULL	1-5 microM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that microtubule interfering agents , paclitaxel ( 1-5 microM ) , colchicine ( 1-100 microM ) , nocodazole ( 1-20 microM ) , and vincristine ( 1-50 microM ) , did not affect either PMA or fMLP-induced oxidative burst .
	manualset3
126213	5	404526	13	NULL	NULL	0	NULL	colchicine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that microtubule interfering agents , paclitaxel ( 1-5 microM ) , colchicine ( 1-100 microM ) , nocodazole ( 1-20 microM ) , and vincristine ( 1-50 microM ) , did not affect either PMA or fMLP-induced oxidative burst .
	manualset3
126214	6	404526	13	NULL	NULL	0	NULL	1-100 microM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that microtubule interfering agents , paclitaxel ( 1-5 microM ) , colchicine ( 1-100 microM ) , nocodazole ( 1-20 microM ) , and vincristine ( 1-50 microM ) , did not affect either PMA or fMLP-induced oxidative burst .
	manualset3
126215	7	404526	13	NULL	NULL	0	NULL	nocodazole 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that microtubule interfering agents , paclitaxel ( 1-5 microM ) , colchicine ( 1-100 microM ) , nocodazole ( 1-20 microM ) , and vincristine ( 1-50 microM ) , did not affect either PMA or fMLP-induced oxidative burst .
	manualset3
126216	8	404526	13	NULL	NULL	0	NULL	1-20 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that microtubule interfering agents , paclitaxel ( 1-5 microM ) , colchicine ( 1-100 microM ) , nocodazole ( 1-20 microM ) , and vincristine ( 1-50 microM ) , did not affect either PMA or fMLP-induced oxidative burst .
	manualset3
126217	9	404526	13	NULL	NULL	0	NULL	vincristine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that microtubule interfering agents , paclitaxel ( 1-5 microM ) , colchicine ( 1-100 microM ) , nocodazole ( 1-20 microM ) , and vincristine ( 1-50 microM ) , did not affect either PMA or fMLP-induced oxidative burst .
	manualset3
126218	10	404526	13	NULL	NULL	0	NULL	1-50 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that microtubule interfering agents , paclitaxel ( 1-5 microM ) , colchicine ( 1-100 microM ) , nocodazole ( 1-20 microM ) , and vincristine ( 1-50 microM ) , did not affect either PMA or fMLP-induced oxidative burst .
	manualset3
126219	11	404526	13	NULL	NULL	0	NULL	PMA-induced oxidative burst	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that microtubule interfering agents , paclitaxel ( 1-5 microM ) , colchicine ( 1-100 microM ) , nocodazole ( 1-20 microM ) , and vincristine ( 1-50 microM ) , did not affect either PMA or fMLP-induced oxidative burst .
	manualset3
126220	12	404526	13	NULL	NULL	0	NULL	fMLP-induced oxidative burst	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that microtubule interfering agents , paclitaxel ( 1-5 microM ) , colchicine ( 1-100 microM ) , nocodazole ( 1-20 microM ) , and vincristine ( 1-50 microM ) , did not affect either PMA or fMLP-induced oxidative burst .
	manualset3
126499	1	404527	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that oxygen free radicals generated by xanthine oxidase and xanthine inhibited strongly the synthesis of DNA , PG and collagen of human embryo chondrocytes .
	manualset3
126500	2	404527	13	NULL	NULL	0	NULL	oxygen free radicals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that oxygen free radicals generated by xanthine oxidase and xanthine inhibited strongly the synthesis of DNA , PG and collagen of human embryo chondrocytes .
	manualset3
126501	3	404527	13	NULL	NULL	0	NULL	xanthine oxidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that oxygen free radicals generated by xanthine oxidase and xanthine inhibited strongly the synthesis of DNA , PG and collagen of human embryo chondrocytes .
	manualset3
126502	4	404527	13	NULL	NULL	0	NULL	xanthine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that oxygen free radicals generated by xanthine oxidase and xanthine inhibited strongly the synthesis of DNA , PG and collagen of human embryo chondrocytes .
	manualset3
126503	5	404527	13	NULL	NULL	0	NULL	synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that oxygen free radicals generated by xanthine oxidase and xanthine inhibited strongly the synthesis of DNA , PG and collagen of human embryo chondrocytes .
	manualset3
126504	6	404527	13	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that oxygen free radicals generated by xanthine oxidase and xanthine inhibited strongly the synthesis of DNA , PG and collagen of human embryo chondrocytes .
	manualset3
126505	7	404527	13	NULL	NULL	0	NULL	PG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that oxygen free radicals generated by xanthine oxidase and xanthine inhibited strongly the synthesis of DNA , PG and collagen of human embryo chondrocytes .
	manualset3
126506	8	404527	13	NULL	NULL	0	NULL	collagen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that oxygen free radicals generated by xanthine oxidase and xanthine inhibited strongly the synthesis of DNA , PG and collagen of human embryo chondrocytes .
	manualset3
126507	9	404527	13	NULL	NULL	0	NULL	human embryo chondrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results showed that oxygen free radicals generated by xanthine oxidase and xanthine inhibited strongly the synthesis of DNA , PG and collagen of human embryo chondrocytes .
	manualset3
126570	1	404528	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest a mechanism for folding in which the formation of a network of interactions among a subset of hydrophobic residues ensures that the native topology is generated .
	manualset3
126571	2	404528	13	NULL	NULL	0	NULL	mechanism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest a mechanism for folding in which the formation of a network of interactions among a subset of hydrophobic residues ensures that the native topology is generated .
	manualset3
126572	3	404528	13	NULL	NULL	0	NULL	formation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest a mechanism for folding in which the formation of a network of interactions among a subset of hydrophobic residues ensures that the native topology is generated .
	manualset3
126573	4	404528	13	NULL	NULL	0	NULL	network of interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest a mechanism for folding in which the formation of a network of interactions among a subset of hydrophobic residues ensures that the native topology is generated .
	manualset3
126574	5	404528	13	NULL	NULL	0	NULL	subset of hydrophobic residues 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest a mechanism for folding in which the formation of a network of interactions among a subset of hydrophobic residues ensures that the native topology is generated .
	manualset3
126576	6	404528	13	NULL	NULL	0	NULL	native topology	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest a mechanism for folding in which the formation of a network of interactions among a subset of hydrophobic residues ensures that the native topology is generated .
	manualset3
126577	1	404529	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest a novel view of the behavior of confined water for models of in vivo protein folding scenarios .
	manualset3
126578	2	404529	13	NULL	NULL	NULL	NULL	novel view	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our results suggest a novel view of the behavior of confined water for models of in vivo protein folding scenarios .
	manualset3
126579	3	404529	13	NULL	NULL	0	NULL	behavior 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest a novel view of the behavior of confined water for models of in vivo protein folding scenarios .
	manualset3
126580	4	404529	13	NULL	NULL	0	NULL	 water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest a novel view of the behavior of confined water for models of in vivo protein folding scenarios .
	manualset3
126581	5	404529	13	NULL	NULL	0	NULL	models 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest a novel view of the behavior of confined water for models of in vivo protein folding scenarios .
	manualset3
126583	6	404529	13	NULL	NULL	0	NULL	protein folding scenarios	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest a novel view of the behavior of confined water for models of in vivo protein folding scenarios .
	manualset3
126584	1	404530	13	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest a previously unknown impact of breastfeeding on the outcome of transplantation .
	manualset3
126585	2	404530	13	NULL	NULL	0	NULL	impact	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest a previously unknown impact of breastfeeding on the outcome of transplantation .
	manualset3
126586	3	404530	13	NULL	NULL	0	NULL	breastfeeding	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest a previously unknown impact of breastfeeding on the outcome of transplantation .
	manualset3
126587	4	404530	13	NULL	NULL	0	NULL	outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest a previously unknown impact of breastfeeding on the outcome of transplantation .
	manualset3
126588	5	404530	13	NULL	NULL	0	NULL	transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest a previously unknown impact of breastfeeding on the outcome of transplantation .
	manualset3
115955	1	404531	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest perceptual and thought disturbance as an important indicator of vulnerability to psychosis .
	manualset3
115956	2	404531	5	NULL	NULL	0	NULL	perceptual disturbance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest perceptual and thought disturbance as an important indicator of vulnerability to psychosis .
	manualset3
115957	3	404531	5	NULL	NULL	0	NULL	thought disturbance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest perceptual and thought disturbance as an important indicator of vulnerability to psychosis .
	manualset3
115958	4	404531	5	NULL	NULL	0	NULL	 important indicator 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest perceptual and thought disturbance as an important indicator of vulnerability to psychosis .
	manualset3
115959	5	404531	5	NULL	NULL	0	NULL	vulnerability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest perceptual and thought disturbance as an important indicator of vulnerability to psychosis .
	manualset3
115960	6	404531	5	NULL	NULL	0	NULL	psychosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest perceptual and thought disturbance as an important indicator of vulnerability to psychosis .
	manualset3
116475	1	404532	5	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that GSCs require the low expression of Cx43 for maintaining their malignant phenotype , and upregulation of Cx43 might be a potential strategy for treatment of malignant glioma .
	manualset3
116476	2	404532	5	NULL	NULL	0	NULL	GSCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that GSCs require the low expression of Cx43 for maintaining their malignant phenotype , and upregulation of Cx43 might be a potential strategy for treatment of malignant glioma .
	manualset3
116477	3	404532	5	NULL	NULL	0	NULL	low expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that GSCs require the low expression of Cx43 for maintaining their malignant phenotype , and upregulation of Cx43 might be a potential strategy for treatment of malignant glioma .
	manualset3
116478	4	404532	5	NULL	NULL	NULL	NULL	Cx43	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our results suggest that GSCs require the low expression of Cx43 for maintaining their malignant phenotype , and upregulation of Cx43 might be a potential strategy for treatment of malignant glioma .
	manualset3
116479	5	404532	5	NULL	NULL	0	NULL	malignant phenotype	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that GSCs require the low expression of Cx43 for maintaining their malignant phenotype , and upregulation of Cx43 might be a potential strategy for treatment of malignant glioma .
	manualset3
116480	6	404532	5	NULL	NULL	0	NULL	upregulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that GSCs require the low expression of Cx43 for maintaining their malignant phenotype , and upregulation of Cx43 might be a potential strategy for treatment of malignant glioma .
	manualset3
116481	7	404532	5	NULL	NULL	0	NULL	Cx43	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that GSCs require the low expression of Cx43 for maintaining their malignant phenotype , and upregulation of Cx43 might be a potential strategy for treatment of malignant glioma .
	manualset3
116482	8	404532	5	NULL	NULL	0	NULL	potential strategy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that GSCs require the low expression of Cx43 for maintaining their malignant phenotype , and upregulation of Cx43 might be a potential strategy for treatment of malignant glioma .
	manualset3
116483	9	404532	5	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that GSCs require the low expression of Cx43 for maintaining their malignant phenotype , and upregulation of Cx43 might be a potential strategy for treatment of malignant glioma .
	manualset3
116484	10	404532	5	NULL	NULL	0	NULL	malignant glioma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that GSCs require the low expression of Cx43 for maintaining their malignant phenotype , and upregulation of Cx43 might be a potential strategy for treatment of malignant glioma .
	manualset3
116485	1	404533	5	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that LIGHT is a costimulatory molecule involved in DC-mediated cellular immune responses .
	manualset3
116486	2	404533	5	NULL	NULL	0	NULL	LIGHT	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that LIGHT is a costimulatory molecule involved in DC-mediated cellular immune responses .
	manualset3
116487	3	404533	5	NULL	NULL	0	NULL	costimulatory molecule	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that LIGHT is a costimulatory molecule involved in DC-mediated cellular immune responses .
	manualset3
116488	4	404533	5	NULL	NULL	NULL	NULL	DC-mediated cellular immune responses	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our results suggest that LIGHT is a costimulatory molecule involved in DC-mediated cellular immune responses .
	manualset3
116489	1	404534	5	NULL	NULL	0	NULL	dynamic model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A dynamic model of plant growth with interactions between development and functional mechanisms to study plant structural plasticity related to trophic competition .
	manualset3
116490	2	404534	5	NULL	NULL	0	NULL	plant growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A dynamic model of plant growth with interactions between development and functional mechanisms to study plant structural plasticity related to trophic competition .
	manualset3
116491	3	404534	5	NULL	NULL	0	NULL	interactions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A dynamic model of plant growth with interactions between development and functional mechanisms to study plant structural plasticity related to trophic competition .
	manualset3
116492	4	404534	5	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A dynamic model of plant growth with interactions between development and functional mechanisms to study plant structural plasticity related to trophic competition .
	manualset3
116493	5	404534	5	NULL	NULL	0	NULL	functional mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A dynamic model of plant growth with interactions between development and functional mechanisms to study plant structural plasticity related to trophic competition .
	manualset3
116494	6	404534	5	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A dynamic model of plant growth with interactions between development and functional mechanisms to study plant structural plasticity related to trophic competition .
	manualset3
116495	7	404534	5	NULL	NULL	0	NULL	plant structural plasticity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A dynamic model of plant growth with interactions between development and functional mechanisms to study plant structural plasticity related to trophic competition .
	manualset3
116496	8	404534	5	NULL	NULL	NULL	NULL	trophic competition	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A dynamic model of plant growth with interactions between development and functional mechanisms to study plant structural plasticity related to trophic competition .
	manualset3
116497	1	404535	5	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that Tsc/mTORC1 signaling and PTEN/PI3K ( phosphatidylinositol 3 kinase ) signaling synergistically regulate the dormancy and activation of primordial follicles , and together ensure the proper length of female reproductive life .
	manualset3
116498	2	404535	5	NULL	NULL	0	NULL	Tsc/mTORC1 signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that Tsc/mTORC1 signaling and PTEN/PI3K ( phosphatidylinositol 3 kinase ) signaling synergistically regulate the dormancy and activation of primordial follicles , and together ensure the proper length of female reproductive life .
	manualset3
116499	3	404535	5	NULL	NULL	0	NULL	PTEN/PI3K ( phosphatidylinositol 3 kinase ) signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that Tsc/mTORC1 signaling and PTEN/PI3K ( phosphatidylinositol 3 kinase ) signaling synergistically regulate the dormancy and activation of primordial follicles , and together ensure the proper length of female reproductive life .
	manualset3
116500	4	404535	5	NULL	NULL	0	NULL	dormancy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that Tsc/mTORC1 signaling and PTEN/PI3K ( phosphatidylinositol 3 kinase ) signaling synergistically regulate the dormancy and activation of primordial follicles , and together ensure the proper length of female reproductive life .
	manualset3
116501	5	404535	5	NULL	NULL	0	NULL	activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that Tsc/mTORC1 signaling and PTEN/PI3K ( phosphatidylinositol 3 kinase ) signaling synergistically regulate the dormancy and activation of primordial follicles , and together ensure the proper length of female reproductive life .
	manualset3
116502	6	404535	5	NULL	NULL	0	NULL	primordial follicles	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that Tsc/mTORC1 signaling and PTEN/PI3K ( phosphatidylinositol 3 kinase ) signaling synergistically regulate the dormancy and activation of primordial follicles , and together ensure the proper length of female reproductive life .
	manualset3
116503	7	404535	5	NULL	NULL	0	NULL	proper length	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that Tsc/mTORC1 signaling and PTEN/PI3K ( phosphatidylinositol 3 kinase ) signaling synergistically regulate the dormancy and activation of primordial follicles , and together ensure the proper length of female reproductive life .
	manualset3
116504	8	404535	5	NULL	NULL	0	NULL	female reproductive life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that Tsc/mTORC1 signaling and PTEN/PI3K ( phosphatidylinositol 3 kinase ) signaling synergistically regulate the dormancy and activation of primordial follicles , and together ensure the proper length of female reproductive life .
	manualset3
116505	1	404536	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that adiponectin could be a positive regulator of the early invasion process by modulating the MMP/TIMP balance .
	manualset3
116506	2	404536	5	NULL	NULL	0	NULL	adiponectin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that adiponectin could be a positive regulator of the early invasion process by modulating the MMP/TIMP balance .
	manualset3
116507	3	404536	5	NULL	NULL	0	NULL	positive regulator	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that adiponectin could be a positive regulator of the early invasion process by modulating the MMP/TIMP balance .
	manualset3
116508	4	404536	5	NULL	NULL	0	NULL	early invasion process	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that adiponectin could be a positive regulator of the early invasion process by modulating the MMP/TIMP balance .
	manualset3
116509	5	404536	5	NULL	NULL	0	NULL	MMP/TIMP balance	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that adiponectin could be a positive regulator of the early invasion process by modulating the MMP/TIMP balance .
	manualset3
116510	1	404537	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that altered placental LCPUFA may result in altered membrane lipid fatty acid composition leading to increased release of sFlt-1 in circulation .
	manualset3
116511	2	404537	5	NULL	NULL	0	NULL	altered placental LCPUFA	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that altered placental LCPUFA may result in altered membrane lipid fatty acid composition leading to increased release of sFlt-1 in circulation .
	manualset3
116512	3	404537	5	NULL	NULL	0	NULL	result 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that altered placental LCPUFA may result in altered membrane lipid fatty acid composition leading to increased release of sFlt-1 in circulation .
	manualset3
116513	4	404537	5	NULL	NULL	0	NULL	membrane lipid fatty acid composition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that altered placental LCPUFA may result in altered membrane lipid fatty acid composition leading to increased release of sFlt-1 in circulation .
	manualset3
116514	5	404537	5	NULL	NULL	NULL	NULL	release 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our results suggest that altered placental LCPUFA may result in altered membrane lipid fatty acid composition leading to increased release of sFlt-1 in circulation .
	manualset3
116515	6	404537	5	NULL	NULL	0	NULL	sFlt-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that altered placental LCPUFA may result in altered membrane lipid fatty acid composition leading to increased release of sFlt-1 in circulation .
	manualset3
116516	7	404537	5	NULL	NULL	0	NULL	circulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that altered placental LCPUFA may result in altered membrane lipid fatty acid composition leading to increased release of sFlt-1 in circulation .
	manualset3
116517	1	404538	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that calcium may lower hip fracture risk in late menopausal women .
	manualset3
116518	2	404538	5	NULL	NULL	0	NULL	calcium 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that calcium may lower hip fracture risk in late menopausal women .
	manualset3
116519	3	404538	5	NULL	NULL	0	NULL	hip fracture risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that calcium may lower hip fracture risk in late menopausal women .
	manualset3
116520	4	404538	5	NULL	NULL	0	NULL	late menopausal women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that calcium may lower hip fracture risk in late menopausal women .
	manualset3
116521	1	404539	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that dexamethasone and insulin stimulate Na , K-ATPase activity in mouse corneal endothelial cells .
	manualset3
116522	2	404539	5	NULL	NULL	0	NULL	dexamethasone 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that dexamethasone and insulin stimulate Na , K-ATPase activity in mouse corneal endothelial cells .
	manualset3
116523	3	404539	5	NULL	NULL	0	NULL	insulin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that dexamethasone and insulin stimulate Na , K-ATPase activity in mouse corneal endothelial cells .
	manualset3
116524	4	404539	5	NULL	NULL	0	NULL	Na , K-ATPase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that dexamethasone and insulin stimulate Na , K-ATPase activity in mouse corneal endothelial cells .
	manualset3
116525	5	404539	5	NULL	NULL	0	NULL	mouse corneal endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that dexamethasone and insulin stimulate Na , K-ATPase activity in mouse corneal endothelial cells .
	manualset3
116526	1	404540	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that divergence has occurred among plant Abc1 family and chloroplast Abc1 kinases play potential roles in regulating dark-induced senescence of plants .
	manualset3
116527	2	404540	5	NULL	NULL	0	NULL	divergence 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that divergence has occurred among plant Abc1 family and chloroplast Abc1 kinases play potential roles in regulating dark-induced senescence of plants .
	manualset3
116528	3	404540	5	NULL	NULL	0	NULL	plant Abc1 family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that divergence has occurred among plant Abc1 family and chloroplast Abc1 kinases play potential roles in regulating dark-induced senescence of plants .
	manualset3
116529	4	404540	5	NULL	NULL	0	NULL	chloroplast Abc1 kinases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that divergence has occurred among plant Abc1 family and chloroplast Abc1 kinases play potential roles in regulating dark-induced senescence of plants .
	manualset3
116530	5	404540	5	NULL	NULL	0	NULL	potential roles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that divergence has occurred among plant Abc1 family and chloroplast Abc1 kinases play potential roles in regulating dark-induced senescence of plants .
	manualset3
116531	6	404540	5	NULL	NULL	0	NULL	dark-induced senescence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that divergence has occurred among plant Abc1 family and chloroplast Abc1 kinases play potential roles in regulating dark-induced senescence of plants .
	manualset3
116532	7	404540	5	NULL	NULL	0	NULL	plants 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that divergence has occurred among plant Abc1 family and chloroplast Abc1 kinases play potential roles in regulating dark-induced senescence of plants .
	manualset3
116533	1	404541	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that genetic variants in DCLK1 are associated with SCZ and , to a lesser extent , with ADHD and BP .
	manualset3
116534	2	404541	5	NULL	NULL	0	NULL	genetic variants	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that genetic variants in DCLK1 are associated with SCZ and , to a lesser extent , with ADHD and BP .
	manualset3
116535	3	404541	5	NULL	NULL	0	NULL	DCLK1 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that genetic variants in DCLK1 are associated with SCZ and , to a lesser extent , with ADHD and BP .
	manualset3
116536	4	404541	5	NULL	NULL	0	NULL	SCZ 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that genetic variants in DCLK1 are associated with SCZ and , to a lesser extent , with ADHD and BP .
	manualset3
116537	5	404541	5	NULL	NULL	0	NULL	ADHD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that genetic variants in DCLK1 are associated with SCZ and , to a lesser extent , with ADHD and BP .
	manualset3
116538	6	404541	5	NULL	NULL	0	NULL	BP	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that genetic variants in DCLK1 are associated with SCZ and , to a lesser extent , with ADHD and BP .
	manualset3
116539	1	404542	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that ingested environmental particles in AM , e.g. , after an episode of high particle concentration , may impair phagocytic capacity of the cells , especially after infections that induce an increased production of IFN-gamma .
	manualset3
116540	2	404542	5	NULL	NULL	0	NULL	ingested environmental particles 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that ingested environmental particles in AM , e.g. , after an episode of high particle concentration , may impair phagocytic capacity of the cells , especially after infections that induce an increased production of IFN-gamma .
	manualset3
116541	3	404542	5	NULL	NULL	0	NULL	AM	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that ingested environmental particles in AM , e.g. , after an episode of high particle concentration , may impair phagocytic capacity of the cells , especially after infections that induce an increased production of IFN-gamma .
	manualset3
116542	4	404542	5	NULL	NULL	0	NULL	episode 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that ingested environmental particles in AM , e.g. , after an episode of high particle concentration , may impair phagocytic capacity of the cells , especially after infections that induce an increased production of IFN-gamma .
	manualset3
116543	5	404542	5	NULL	NULL	0	NULL	high particle concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that ingested environmental particles in AM , e.g. , after an episode of high particle concentration , may impair phagocytic capacity of the cells , especially after infections that induce an increased production of IFN-gamma .
	manualset3
116544	6	404542	5	NULL	NULL	0	NULL	phagocytic capacity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that ingested environmental particles in AM , e.g. , after an episode of high particle concentration , may impair phagocytic capacity of the cells , especially after infections that induce an increased production of IFN-gamma .
	manualset3
116545	7	404542	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that ingested environmental particles in AM , e.g. , after an episode of high particle concentration , may impair phagocytic capacity of the cells , especially after infections that induce an increased production of IFN-gamma .
	manualset3
116546	8	404542	5	NULL	NULL	0	NULL	infections 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that ingested environmental particles in AM , e.g. , after an episode of high particle concentration , may impair phagocytic capacity of the cells , especially after infections that induce an increased production of IFN-gamma .
	manualset3
116547	9	404542	5	NULL	NULL	0	NULL	increased production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that ingested environmental particles in AM , e.g. , after an episode of high particle concentration , may impair phagocytic capacity of the cells , especially after infections that induce an increased production of IFN-gamma .
	manualset3
116548	10	404542	5	NULL	NULL	0	NULL	IFN-gamma 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that ingested environmental particles in AM , e.g. , after an episode of high particle concentration , may impair phagocytic capacity of the cells , especially after infections that induce an increased production of IFN-gamma .
	manualset3
116549	1	404543	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that local adaptation is less common in plant populations than generally assumed .
	manualset3
116550	2	404543	5	NULL	NULL	0	NULL	local adaptation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that local adaptation is less common in plant populations than generally assumed .
	manualset3
116551	3	404543	5	NULL	NULL	0	NULL	plant populations	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that local adaptation is less common in plant populations than generally assumed .
	manualset3
116552	1	404544	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that mTOR , p38 , and JNK play important roles in VEGF-C expression , and that rapamycin has an antilymphangiogentic effect and exerts the expected inhibition of lymphatic metastasis .
	manualset3
116553	2	404544	5	NULL	NULL	0	NULL	mTOR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that mTOR , p38 , and JNK play important roles in VEGF-C expression , and that rapamycin has an antilymphangiogentic effect and exerts the expected inhibition of lymphatic metastasis .
	manualset3
116554	3	404544	5	NULL	NULL	0	NULL	p38	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that mTOR , p38 , and JNK play important roles in VEGF-C expression , and that rapamycin has an antilymphangiogentic effect and exerts the expected inhibition of lymphatic metastasis .
	manualset3
116555	4	404544	5	NULL	NULL	0	NULL	JNK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that mTOR , p38 , and JNK play important roles in VEGF-C expression , and that rapamycin has an antilymphangiogentic effect and exerts the expected inhibition of lymphatic metastasis .
	manualset3
116556	5	404544	5	NULL	NULL	0	NULL	important roles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that mTOR , p38 , and JNK play important roles in VEGF-C expression , and that rapamycin has an antilymphangiogentic effect and exerts the expected inhibition of lymphatic metastasis .
	manualset3
116557	6	404544	5	NULL	NULL	0	NULL	VEGF-C expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that mTOR , p38 , and JNK play important roles in VEGF-C expression , and that rapamycin has an antilymphangiogentic effect and exerts the expected inhibition of lymphatic metastasis .
	manualset3
116558	7	404544	5	NULL	NULL	0	NULL	rapamycin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that mTOR , p38 , and JNK play important roles in VEGF-C expression , and that rapamycin has an antilymphangiogentic effect and exerts the expected inhibition of lymphatic metastasis .
	manualset3
116559	8	404544	5	NULL	NULL	0	NULL	antilymphangiogentic effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that mTOR , p38 , and JNK play important roles in VEGF-C expression , and that rapamycin has an antilymphangiogentic effect and exerts the expected inhibition of lymphatic metastasis .
	manualset3
116560	9	404544	5	NULL	NULL	0	NULL	inhibition 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that mTOR , p38 , and JNK play important roles in VEGF-C expression , and that rapamycin has an antilymphangiogentic effect and exerts the expected inhibition of lymphatic metastasis .
	manualset3
116561	10	404544	5	NULL	NULL	0	NULL	lymphatic metastasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that mTOR , p38 , and JNK play important roles in VEGF-C expression , and that rapamycin has an antilymphangiogentic effect and exerts the expected inhibition of lymphatic metastasis .
	manualset3
116562	1	404545	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that multiple Su ( var ) 3-9 family members are active in Arabidopsis and that dimethylation of histone H3 lysine 9 is the critical mark for gene silencing and DNA methylation .
	manualset3
116563	2	404545	5	NULL	NULL	0	NULL	multiple Su ( var ) 3-9 family members 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that multiple Su ( var ) 3-9 family members are active in Arabidopsis and that dimethylation of histone H3 lysine 9 is the critical mark for gene silencing and DNA methylation .
	manualset3
116564	3	404545	5	NULL	NULL	0	NULL	Arabidopsis 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that multiple Su ( var ) 3-9 family members are active in Arabidopsis and that dimethylation of histone H3 lysine 9 is the critical mark for gene silencing and DNA methylation .
	manualset3
116565	4	404545	5	NULL	NULL	0	NULL	dimethylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that multiple Su ( var ) 3-9 family members are active in Arabidopsis and that dimethylation of histone H3 lysine 9 is the critical mark for gene silencing and DNA methylation .
	manualset3
116566	5	404545	5	NULL	NULL	0	NULL	histone H3 lysine 9	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that multiple Su ( var ) 3-9 family members are active in Arabidopsis and that dimethylation of histone H3 lysine 9 is the critical mark for gene silencing and DNA methylation .
	manualset3
116567	6	404545	5	NULL	NULL	0	NULL	critical mark	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that multiple Su ( var ) 3-9 family members are active in Arabidopsis and that dimethylation of histone H3 lysine 9 is the critical mark for gene silencing and DNA methylation .
	manualset3
116568	7	404545	5	NULL	NULL	0	NULL	gene silencing	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that multiple Su ( var ) 3-9 family members are active in Arabidopsis and that dimethylation of histone H3 lysine 9 is the critical mark for gene silencing and DNA methylation .
	manualset3
116569	8	404545	5	NULL	NULL	0	NULL	DNA methylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that multiple Su ( var ) 3-9 family members are active in Arabidopsis and that dimethylation of histone H3 lysine 9 is the critical mark for gene silencing and DNA methylation .
	manualset3
116570	1	404546	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that multiple contacts between NCoA-1 , CBP , and STAT6 are required for transcriptional activation .
	manualset3
116571	2	404546	5	NULL	NULL	0	NULL	multiple contacts	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that multiple contacts between NCoA-1 , CBP , and STAT6 are required for transcriptional activation .
	manualset3
116572	3	404546	5	NULL	NULL	0	NULL	 NCoA-1	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that multiple contacts between NCoA-1 , CBP , and STAT6 are required for transcriptional activation .
	manualset3
116573	4	404546	5	NULL	NULL	0	NULL	CBP 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that multiple contacts between NCoA-1 , CBP , and STAT6 are required for transcriptional activation .
	manualset3
116574	5	404546	5	NULL	NULL	0	NULL	STAT6 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that multiple contacts between NCoA-1 , CBP , and STAT6 are required for transcriptional activation .
	manualset3
116575	6	404546	5	NULL	NULL	0	NULL	transcriptional activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that multiple contacts between NCoA-1 , CBP , and STAT6 are required for transcriptional activation .
	manualset3
116576	1	404547	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that radical orchiectomy should not be performed indiscriminately in all patients with testicular lesions that are sonographically suspicious for neoplasm .
	manualset3
116577	2	404547	5	NULL	NULL	0	NULL	radical orchiectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that radical orchiectomy should not be performed indiscriminately in all patients with testicular lesions that are sonographically suspicious for neoplasm .
	manualset3
116578	3	404547	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that radical orchiectomy should not be performed indiscriminately in all patients with testicular lesions that are sonographically suspicious for neoplasm .
	manualset3
116579	4	404547	5	NULL	NULL	0	NULL	testicular lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that radical orchiectomy should not be performed indiscriminately in all patients with testicular lesions that are sonographically suspicious for neoplasm .
	manualset3
116580	5	404547	5	NULL	NULL	0	NULL	neoplasm 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that radical orchiectomy should not be performed indiscriminately in all patients with testicular lesions that are sonographically suspicious for neoplasm .
	manualset3
116581	1	404548	5	NULL	NULL	0	NULL	results 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that selective intestinal decontamination may be useful as a prophylactic measure against spontaneous bacterial peritonitis in those patients with liver cirrhosis at high risk of infection by increasing the bactericidal capacity of ascitic fluid .
	manualset3
116582	2	404548	5	NULL	NULL	0	NULL	selective intestinal decontamination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that selective intestinal decontamination may be useful as a prophylactic measure against spontaneous bacterial peritonitis in those patients with liver cirrhosis at high risk of infection by increasing the bactericidal capacity of ascitic fluid .
	manualset3
116583	3	404548	5	NULL	NULL	0	NULL	prophylactic measure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that selective intestinal decontamination may be useful as a prophylactic measure against spontaneous bacterial peritonitis in those patients with liver cirrhosis at high risk of infection by increasing the bactericidal capacity of ascitic fluid .
	manualset3
116584	4	404548	5	NULL	NULL	0	NULL	spontaneous bacterial peritonitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that selective intestinal decontamination may be useful as a prophylactic measure against spontaneous bacterial peritonitis in those patients with liver cirrhosis at high risk of infection by increasing the bactericidal capacity of ascitic fluid .
	manualset3
116585	5	404548	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that selective intestinal decontamination may be useful as a prophylactic measure against spontaneous bacterial peritonitis in those patients with liver cirrhosis at high risk of infection by increasing the bactericidal capacity of ascitic fluid .
	manualset3
116586	6	404548	5	NULL	NULL	0	NULL	liver cirrhosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that selective intestinal decontamination may be useful as a prophylactic measure against spontaneous bacterial peritonitis in those patients with liver cirrhosis at high risk of infection by increasing the bactericidal capacity of ascitic fluid .
	manualset3
116587	7	404548	5	NULL	NULL	0	NULL	high risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that selective intestinal decontamination may be useful as a prophylactic measure against spontaneous bacterial peritonitis in those patients with liver cirrhosis at high risk of infection by increasing the bactericidal capacity of ascitic fluid .
	manualset3
116588	8	404548	5	NULL	NULL	0	NULL	infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that selective intestinal decontamination may be useful as a prophylactic measure against spontaneous bacterial peritonitis in those patients with liver cirrhosis at high risk of infection by increasing the bactericidal capacity of ascitic fluid .
	manualset3
116589	9	404548	5	NULL	NULL	0	NULL	bactericidal capacity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that selective intestinal decontamination may be useful as a prophylactic measure against spontaneous bacterial peritonitis in those patients with liver cirrhosis at high risk of infection by increasing the bactericidal capacity of ascitic fluid .
	manualset3
116590	10	404548	5	NULL	NULL	0	NULL	ascitic fluid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that selective intestinal decontamination may be useful as a prophylactic measure against spontaneous bacterial peritonitis in those patients with liver cirrhosis at high risk of infection by increasing the bactericidal capacity of ascitic fluid .
	manualset3
116591	1	404549	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that seropositivity to antibodies against Nepsilon-homocysteinylated albumin is associated with early-onset CAD .
	manualset3
116592	2	404549	5	NULL	NULL	0	NULL	seropositivity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that seropositivity to antibodies against Nepsilon-homocysteinylated albumin is associated with early-onset CAD .
	manualset3
116593	3	404549	5	NULL	NULL	0	NULL	antibodies against Nepsilon-homocysteinylated albumin	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that seropositivity to antibodies against Nepsilon-homocysteinylated albumin is associated with early-onset CAD .
	manualset3
116594	4	404549	5	NULL	NULL	0	NULL	early-onset CAD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that seropositivity to antibodies against Nepsilon-homocysteinylated albumin is associated with early-onset CAD .
	manualset3
116595	1	404550	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that the G-C-rich regions have to be positioned between the enhancer element and the initiation sites to stimulate transcription from downstream sites .
	manualset3
116596	2	404550	5	NULL	NULL	0	NULL	G-C-rich regions	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that the G-C-rich regions have to be positioned between the enhancer element and the initiation sites to stimulate transcription from downstream sites .
	manualset3
116597	3	404550	5	NULL	NULL	0	NULL	enhancer element	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that the G-C-rich regions have to be positioned between the enhancer element and the initiation sites to stimulate transcription from downstream sites .
	manualset3
116598	4	404550	5	NULL	NULL	0	NULL	initiation sites	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that the G-C-rich regions have to be positioned between the enhancer element and the initiation sites to stimulate transcription from downstream sites .
	manualset3
116599	5	404550	5	NULL	NULL	0	NULL	transcription 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that the G-C-rich regions have to be positioned between the enhancer element and the initiation sites to stimulate transcription from downstream sites .
	manualset3
116600	6	404550	5	NULL	NULL	0	NULL	downstream sites	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that the G-C-rich regions have to be positioned between the enhancer element and the initiation sites to stimulate transcription from downstream sites .
	manualset3
116601	1	404551	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that the low discriminating ability observed in some parasitic wasps could probably be an evolutionary response to host defences pressure .
	manualset3
116602	2	404551	5	NULL	NULL	0	NULL	discriminating ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that the low discriminating ability observed in some parasitic wasps could probably be an evolutionary response to host defences pressure .
	manualset3
116603	3	404551	5	NULL	NULL	0	NULL	parasitic wasps	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that the low discriminating ability observed in some parasitic wasps could probably be an evolutionary response to host defences pressure .
	manualset3
116604	4	404551	5	NULL	NULL	0	NULL	evolutionary response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that the low discriminating ability observed in some parasitic wasps could probably be an evolutionary response to host defences pressure .
	manualset3
116605	5	404551	5	NULL	NULL	0	NULL	host defences pressure	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results suggest that the low discriminating ability observed in some parasitic wasps could probably be an evolutionary response to host defences pressure .
	manualset3
116606	1	404552	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results support that the molecular structure of the VNTR allele , not only its overall length , is associated with variations of insulin secretion .
	manualset3
116607	2	404552	5	NULL	NULL	0	NULL	molecular structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results support that the molecular structure of the VNTR allele , not only its overall length , is associated with variations of insulin secretion .
	manualset3
116608	3	404552	5	NULL	NULL	0	NULL	VNTR allele	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results support that the molecular structure of the VNTR allele , not only its overall length , is associated with variations of insulin secretion .
	manualset3
116609	4	404552	5	NULL	NULL	0	NULL	length 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results support that the molecular structure of the VNTR allele , not only its overall length , is associated with variations of insulin secretion .
	manualset3
116610	5	404552	5	NULL	NULL	0	NULL	variations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results support that the molecular structure of the VNTR allele , not only its overall length , is associated with variations of insulin secretion .
	manualset3
116611	6	404552	5	NULL	NULL	0	NULL	insulin secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results support that the molecular structure of the VNTR allele , not only its overall length , is associated with variations of insulin secretion .
	manualset3
116612	1	404553	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results support the hypothesis that hyperinsulinemia may play a role in colorectal carcinogenesis , even in a relatively lean population .
	manualset3
116613	2	404553	5	NULL	NULL	0	NULL	hypothesis 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results support the hypothesis that hyperinsulinemia may play a role in colorectal carcinogenesis , even in a relatively lean population .
	manualset3
116614	3	404553	5	NULL	NULL	0	NULL	hyperinsulinemia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results support the hypothesis that hyperinsulinemia may play a role in colorectal carcinogenesis , even in a relatively lean population .
	manualset3
116615	4	404553	5	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results support the hypothesis that hyperinsulinemia may play a role in colorectal carcinogenesis , even in a relatively lean population .
	manualset3
116616	5	404553	5	NULL	NULL	0	NULL	colorectal carcinogenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results support the hypothesis that hyperinsulinemia may play a role in colorectal carcinogenesis , even in a relatively lean population .
	manualset3
116617	6	404553	5	NULL	NULL	0	NULL	relatively lean population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results support the hypothesis that hyperinsulinemia may play a role in colorectal carcinogenesis , even in a relatively lean population .
	manualset3
116618	1	404554	5	NULL	NULL	0	NULL	factor analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A factor analysis of the Reminiscence Uses Scale yielded three factor subscales : Self-Regard/Image Enhancement , Present Problem Solving , and Existential/Self-Understanding .
	manualset3
116619	2	404554	5	NULL	NULL	0	NULL	Reminiscence Uses Scale	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A factor analysis of the Reminiscence Uses Scale yielded three factor subscales : Self-Regard/Image Enhancement , Present Problem Solving , and Existential/Self-Understanding .
	manualset3
116620	3	404554	5	NULL	NULL	0	NULL	three factor subscales	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A factor analysis of the Reminiscence Uses Scale yielded three factor subscales : Self-Regard/Image Enhancement , Present Problem Solving , and Existential/Self-Understanding .
	manualset3
116621	4	404554	5	NULL	NULL	0	NULL	Self-Regard/Image Enhancement	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A factor analysis of the Reminiscence Uses Scale yielded three factor subscales : Self-Regard/Image Enhancement , Present Problem Solving , and Existential/Self-Understanding .
	manualset3
116622	5	404554	5	NULL	NULL	0	NULL	Present Problem Solving	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A factor analysis of the Reminiscence Uses Scale yielded three factor subscales : Self-Regard/Image Enhancement , Present Problem Solving , and Existential/Self-Understanding .
	manualset3
116623	6	404554	5	NULL	NULL	0	NULL	Existential/Self-Understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A factor analysis of the Reminiscence Uses Scale yielded three factor subscales : Self-Regard/Image Enhancement , Present Problem Solving , and Existential/Self-Understanding .
	manualset3
116624	1	404555	5	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies provide evidence that peroxisomal ABC transporters utilize ATP to become a functional transporter and that ALD gene mutations alter peroxisomal transport function .
	manualset3
116625	2	404555	5	NULL	NULL	0	NULL	evidence 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies provide evidence that peroxisomal ABC transporters utilize ATP to become a functional transporter and that ALD gene mutations alter peroxisomal transport function .
	manualset3
116626	3	404555	5	NULL	NULL	0	NULL	peroxisomal ABC transporters	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies provide evidence that peroxisomal ABC transporters utilize ATP to become a functional transporter and that ALD gene mutations alter peroxisomal transport function .
	manualset3
116627	4	404555	5	NULL	NULL	0	NULL	ATP 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies provide evidence that peroxisomal ABC transporters utilize ATP to become a functional transporter and that ALD gene mutations alter peroxisomal transport function .
	manualset3
116628	5	404555	5	NULL	NULL	0	NULL	functional transporter	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies provide evidence that peroxisomal ABC transporters utilize ATP to become a functional transporter and that ALD gene mutations alter peroxisomal transport function .
	manualset3
116629	6	404555	5	NULL	NULL	0	NULL	ALD gene mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies provide evidence that peroxisomal ABC transporters utilize ATP to become a functional transporter and that ALD gene mutations alter peroxisomal transport function .
	manualset3
116630	7	404555	5	NULL	NULL	0	NULL	peroxisomal transport function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies provide evidence that peroxisomal ABC transporters utilize ATP to become a functional transporter and that ALD gene mutations alter peroxisomal transport function .
	manualset3
116631	1	404556	5	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies showed that the dissolution rate of evodiamine was significantly higher in the solid dispersion system in comparison with that in enriched samples of evodiamine or physical mixtures .
	manualset3
116632	2	404556	5	NULL	NULL	0	NULL	dissolution rate 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies showed that the dissolution rate of evodiamine was significantly higher in the solid dispersion system in comparison with that in enriched samples of evodiamine or physical mixtures .
	manualset3
116633	3	404556	5	NULL	NULL	0	NULL	evodiamine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies showed that the dissolution rate of evodiamine was significantly higher in the solid dispersion system in comparison with that in enriched samples of evodiamine or physical mixtures .
	manualset3
116634	4	404556	5	NULL	NULL	0	NULL	solid dispersion system	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies showed that the dissolution rate of evodiamine was significantly higher in the solid dispersion system in comparison with that in enriched samples of evodiamine or physical mixtures .
	manualset3
116635	5	404556	5	NULL	NULL	0	NULL	comparison 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies showed that the dissolution rate of evodiamine was significantly higher in the solid dispersion system in comparison with that in enriched samples of evodiamine or physical mixtures .
	manualset3
116636	6	404556	5	NULL	NULL	0	NULL	enriched samples	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies showed that the dissolution rate of evodiamine was significantly higher in the solid dispersion system in comparison with that in enriched samples of evodiamine or physical mixtures .
	manualset3
116637	7	404556	5	NULL	NULL	0	NULL	evodiamine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies showed that the dissolution rate of evodiamine was significantly higher in the solid dispersion system in comparison with that in enriched samples of evodiamine or physical mixtures .
	manualset3
116638	8	404556	5	NULL	NULL	0	NULL	physical mixtures	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies showed that the dissolution rate of evodiamine was significantly higher in the solid dispersion system in comparison with that in enriched samples of evodiamine or physical mixtures .
	manualset3
116639	1	404557	5	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies suggest that oncogenic fusion proteins that retain the DBD of the transcription factor ( TF ) and the multimerization sequence of the partner protein can act in a DN manner by multimerizing and binding avidly to gene targets , preventing the normal TF from binding and inducing expression of its target genes .
	manualset3
116640	2	404557	5	NULL	NULL	0	NULL	oncogenic fusion proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies suggest that oncogenic fusion proteins that retain the DBD of the transcription factor ( TF ) and the multimerization sequence of the partner protein can act in a DN manner by multimerizing and binding avidly to gene targets , preventing the normal TF from binding and inducing expression of its target genes .
	manualset3
116641	3	404557	5	NULL	NULL	0	NULL	DBD	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies suggest that oncogenic fusion proteins that retain the DBD of the transcription factor ( TF ) and the multimerization sequence of the partner protein can act in a DN manner by multimerizing and binding avidly to gene targets , preventing the normal TF from binding and inducing expression of its target genes .
	manualset3
116642	4	404557	5	NULL	NULL	0	NULL	transcription factor ( TF )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies suggest that oncogenic fusion proteins that retain the DBD of the transcription factor ( TF ) and the multimerization sequence of the partner protein can act in a DN manner by multimerizing and binding avidly to gene targets , preventing the normal TF from binding and inducing expression of its target genes .
	manualset3
116643	5	404557	5	NULL	NULL	0	NULL	multimerization sequence	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies suggest that oncogenic fusion proteins that retain the DBD of the transcription factor ( TF ) and the multimerization sequence of the partner protein can act in a DN manner by multimerizing and binding avidly to gene targets , preventing the normal TF from binding and inducing expression of its target genes .
	manualset3
116644	6	404557	5	NULL	NULL	0	NULL	partner protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies suggest that oncogenic fusion proteins that retain the DBD of the transcription factor ( TF ) and the multimerization sequence of the partner protein can act in a DN manner by multimerizing and binding avidly to gene targets , preventing the normal TF from binding and inducing expression of its target genes .
	manualset3
116645	7	404557	5	NULL	NULL	0	NULL	DN manner	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies suggest that oncogenic fusion proteins that retain the DBD of the transcription factor ( TF ) and the multimerization sequence of the partner protein can act in a DN manner by multimerizing and binding avidly to gene targets , preventing the normal TF from binding and inducing expression of its target genes .
	manualset3
116646	8	404557	5	NULL	NULL	0	NULL	gene targets	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies suggest that oncogenic fusion proteins that retain the DBD of the transcription factor ( TF ) and the multimerization sequence of the partner protein can act in a DN manner by multimerizing and binding avidly to gene targets , preventing the normal TF from binding and inducing expression of its target genes .
	manualset3
116647	9	404557	5	NULL	NULL	0	NULL	normal TF 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies suggest that oncogenic fusion proteins that retain the DBD of the transcription factor ( TF ) and the multimerization sequence of the partner protein can act in a DN manner by multimerizing and binding avidly to gene targets , preventing the normal TF from binding and inducing expression of its target genes .
	manualset3
116648	10	404557	5	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies suggest that oncogenic fusion proteins that retain the DBD of the transcription factor ( TF ) and the multimerization sequence of the partner protein can act in a DN manner by multimerizing and binding avidly to gene targets , preventing the normal TF from binding and inducing expression of its target genes .
	manualset3
116649	11	404557	5	NULL	NULL	0	NULL	target genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies suggest that oncogenic fusion proteins that retain the DBD of the transcription factor ( TF ) and the multimerization sequence of the partner protein can act in a DN manner by multimerizing and binding avidly to gene targets , preventing the normal TF from binding and inducing expression of its target genes .
	manualset3
116650	1	404558	5	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies suggest that p21Cip1/Waf1 stability may determine G1 arrest duration and that premature degradation of this protein could provide an alternative route to subversion of the G1 checkpoint in cancer cells .
	manualset3
116651	2	404558	5	NULL	NULL	0	NULL	p21Cip1/Waf1 stability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies suggest that p21Cip1/Waf1 stability may determine G1 arrest duration and that premature degradation of this protein could provide an alternative route to subversion of the G1 checkpoint in cancer cells .
	manualset3
116652	3	404558	5	NULL	NULL	0	NULL	 G1 arrest duration 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies suggest that p21Cip1/Waf1 stability may determine G1 arrest duration and that premature degradation of this protein could provide an alternative route to subversion of the G1 checkpoint in cancer cells .
	manualset3
116653	4	404558	5	NULL	NULL	0	NULL	premature degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies suggest that p21Cip1/Waf1 stability may determine G1 arrest duration and that premature degradation of this protein could provide an alternative route to subversion of the G1 checkpoint in cancer cells .
	manualset3
116654	5	404558	5	NULL	NULL	0	NULL	protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies suggest that p21Cip1/Waf1 stability may determine G1 arrest duration and that premature degradation of this protein could provide an alternative route to subversion of the G1 checkpoint in cancer cells .
	manualset3
116655	6	404558	5	NULL	NULL	0	NULL	alternative route	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies suggest that p21Cip1/Waf1 stability may determine G1 arrest duration and that premature degradation of this protein could provide an alternative route to subversion of the G1 checkpoint in cancer cells .
	manualset3
116656	7	404558	5	NULL	NULL	0	NULL	subversion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies suggest that p21Cip1/Waf1 stability may determine G1 arrest duration and that premature degradation of this protein could provide an alternative route to subversion of the G1 checkpoint in cancer cells .
	manualset3
116657	8	404558	5	NULL	NULL	NULL	NULL	G1 checkpoint	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our studies suggest that p21Cip1/Waf1 stability may determine G1 arrest duration and that premature degradation of this protein could provide an alternative route to subversion of the G1 checkpoint in cancer cells .
	manualset3
116658	9	404558	5	NULL	NULL	0	NULL	cancer cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies suggest that p21Cip1/Waf1 stability may determine G1 arrest duration and that premature degradation of this protein could provide an alternative route to subversion of the G1 checkpoint in cancer cells .
	manualset3
116659	1	404559	5	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies suggest that therapy with replicating MV stimulates a strong neutrophil antitumor response , which can be cytokine-enhanced to improve oncolysis .
	manualset3
116660	2	404559	5	NULL	NULL	0	NULL	therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies suggest that therapy with replicating MV stimulates a strong neutrophil antitumor response , which can be cytokine-enhanced to improve oncolysis .
	manualset3
116661	3	404559	5	NULL	NULL	0	NULL	replicating MV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies suggest that therapy with replicating MV stimulates a strong neutrophil antitumor response , which can be cytokine-enhanced to improve oncolysis .
	manualset3
116662	4	404559	5	NULL	NULL	0	NULL	strong neutrophil antitumor response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies suggest that therapy with replicating MV stimulates a strong neutrophil antitumor response , which can be cytokine-enhanced to improve oncolysis .
	manualset3
116663	5	404559	5	NULL	NULL	0	NULL	oncolysis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies suggest that therapy with replicating MV stimulates a strong neutrophil antitumor response , which can be cytokine-enhanced to improve oncolysis .
	manualset3
116664	1	404560	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study explored a largely unacknowledged obstacle to abortion access in Massachusetts : the unwillingness of nurses to staff abortion procedures .
	manualset3
116665	2	404560	5	NULL	NULL	0	NULL	largely unacknowledged obstacle 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study explored a largely unacknowledged obstacle to abortion access in Massachusetts : the unwillingness of nurses to staff abortion procedures .
	manualset3
116666	3	404560	5	NULL	NULL	0	NULL	abortion access	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study explored a largely unacknowledged obstacle to abortion access in Massachusetts : the unwillingness of nurses to staff abortion procedures .
	manualset3
116667	4	404560	5	NULL	NULL	0	NULL	Massachusetts 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study explored a largely unacknowledged obstacle to abortion access in Massachusetts : the unwillingness of nurses to staff abortion procedures .
	manualset3
116668	5	404560	5	NULL	NULL	0	NULL	unwillingness 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study explored a largely unacknowledged obstacle to abortion access in Massachusetts : the unwillingness of nurses to staff abortion procedures .
	manualset3
116669	6	404560	5	NULL	NULL	0	NULL	nurses 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study explored a largely unacknowledged obstacle to abortion access in Massachusetts : the unwillingness of nurses to staff abortion procedures .
	manualset3
116670	7	404560	5	NULL	NULL	0	NULL	abortion procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study explored a largely unacknowledged obstacle to abortion access in Massachusetts : the unwillingness of nurses to staff abortion procedures .
	manualset3
116671	1	404561	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study indicated that eNOS T allele interacts with MTHFR variants , especially MTHFR A1298C to increase the risk of macroalbuminuria and progression from micro-to macro-albuminuria .
	manualset3
116672	2	404561	5	NULL	NULL	NULL	NULL	eNOS T allele	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our study indicated that eNOS T allele interacts with MTHFR variants , especially MTHFR A1298C to increase the risk of macroalbuminuria and progression from micro-to macro-albuminuria .
	manualset3
116673	3	404561	5	NULL	NULL	0	NULL	MTHFR variants	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study indicated that eNOS T allele interacts with MTHFR variants , especially MTHFR A1298C to increase the risk of macroalbuminuria and progression from micro-to macro-albuminuria .
	manualset3
116674	4	404561	5	NULL	NULL	NULL	NULL	MTHFR A1298C 	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our study indicated that eNOS T allele interacts with MTHFR variants , especially MTHFR A1298C to increase the risk of macroalbuminuria and progression from micro-to macro-albuminuria .
	manualset3
116675	5	404561	5	NULL	NULL	0	NULL	risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study indicated that eNOS T allele interacts with MTHFR variants , especially MTHFR A1298C to increase the risk of macroalbuminuria and progression from micro-to macro-albuminuria .
	manualset3
116676	6	404561	5	NULL	NULL	NULL	NULL	macroalbuminuria 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our study indicated that eNOS T allele interacts with MTHFR variants , especially MTHFR A1298C to increase the risk of macroalbuminuria and progression from micro-to macro-albuminuria .
	manualset3
116677	7	404561	5	NULL	NULL	0	NULL	progression 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study indicated that eNOS T allele interacts with MTHFR variants , especially MTHFR A1298C to increase the risk of macroalbuminuria and progression from micro-to macro-albuminuria .
	manualset3
116678	8	404561	5	NULL	NULL	0	NULL	micro-albuminuria 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study indicated that eNOS T allele interacts with MTHFR variants , especially MTHFR A1298C to increase the risk of macroalbuminuria and progression from micro-to macro-albuminuria .
	manualset3
116679	9	404561	5	NULL	NULL	0	NULL	macro-albuminuria 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study indicated that eNOS T allele interacts with MTHFR variants , especially MTHFR A1298C to increase the risk of macroalbuminuria and progression from micro-to macro-albuminuria .
	manualset3
116680	1	404562	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study showed a high level of satisfaction among all users of a store-and-forward teledermatology consult system , and , in some cases , our survey results could be validated with observed clinical outcomes .
	manualset3
116681	2	404562	5	NULL	NULL	0	NULL	high level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study showed a high level of satisfaction among all users of a store-and-forward teledermatology consult system , and , in some cases , our survey results could be validated with observed clinical outcomes .
	manualset3
116682	3	404562	5	NULL	NULL	0	NULL	satisfaction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study showed a high level of satisfaction among all users of a store-and-forward teledermatology consult system , and , in some cases , our survey results could be validated with observed clinical outcomes .
	manualset3
116683	4	404562	5	NULL	NULL	0	NULL	users 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study showed a high level of satisfaction among all users of a store-and-forward teledermatology consult system , and , in some cases , our survey results could be validated with observed clinical outcomes .
	manualset3
116684	5	404562	5	NULL	NULL	0	NULL	store-and-forward teledermatology consult system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study showed a high level of satisfaction among all users of a store-and-forward teledermatology consult system , and , in some cases , our survey results could be validated with observed clinical outcomes .
	manualset3
116685	6	404562	5	NULL	NULL	0	NULL	cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study showed a high level of satisfaction among all users of a store-and-forward teledermatology consult system , and , in some cases , our survey results could be validated with observed clinical outcomes .
	manualset3
116686	7	404562	5	NULL	NULL	NULL	NULL	survey results	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our study showed a high level of satisfaction among all users of a store-and-forward teledermatology consult system , and , in some cases , our survey results could be validated with observed clinical outcomes .
	manualset3
116687	8	404562	5	NULL	NULL	0	NULL	observed clinical outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study showed a high level of satisfaction among all users of a store-and-forward teledermatology consult system , and , in some cases , our survey results could be validated with observed clinical outcomes .
	manualset3
116688	1	404563	5	NULL	NULL	0	NULL	administration 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our administration reasonably assumed that existing employees would be galvanized into PACS personnel .
	manualset3
116689	2	404563	5	NULL	NULL	0	NULL	existing employees	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our administration reasonably assumed that existing employees would be galvanized into PACS personnel .
	manualset3
116690	3	404563	5	NULL	NULL	0	NULL	 PACS personnel	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our administration reasonably assumed that existing employees would be galvanized into PACS personnel .
	manualset3
116691	1	404564	5	NULL	NULL	0	NULL	algorithm 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Our algorithm is available at http : //www-micrel.deis.unibo.it/~tom/ .
	manualset3
116692	1	404565	5	NULL	NULL	0	NULL	analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our analysis also shows that population divergence is most marked after the age of 9 years , with a peak difference seen at age 10 .
	manualset3
116693	2	404565	5	NULL	NULL	0	NULL	population divergence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our analysis also shows that population divergence is most marked after the age of 9 years , with a peak difference seen at age 10 .
	manualset3
116694	3	404565	5	NULL	NULL	0	NULL	age 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Our analysis also shows that population divergence is most marked after the age of 9 years , with a peak difference seen at age 10 .
	manualset3
116695	4	404565	5	NULL	NULL	0	NULL	9 years	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Our analysis also shows that population divergence is most marked after the age of 9 years , with a peak difference seen at age 10 .
	manualset3
116696	5	404565	5	NULL	NULL	0	NULL	peak difference	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our analysis also shows that population divergence is most marked after the age of 9 years , with a peak difference seen at age 10 .
	manualset3
116697	6	404565	5	NULL	NULL	0	NULL	age 10	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Our analysis also shows that population divergence is most marked after the age of 9 years , with a peak difference seen at age 10 .
	manualset3
116698	1	404566	5	NULL	NULL	0	NULL	factor 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A factor was discovered in the human serum , placental serum from the umbilical cord of pregnant women and sera of peripheral blood from some healthy donors , which induces one of the late stages of differentiation : switching of IgM to IgG synthesis in the RPMI-6410t line of human lymphoblastoid B-cells .
	manualset3
116699	2	404566	5	NULL	NULL	0	NULL	human serum	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A factor was discovered in the human serum , placental serum from the umbilical cord of pregnant women and sera of peripheral blood from some healthy donors , which induces one of the late stages of differentiation : switching of IgM to IgG synthesis in the RPMI-6410t line of human lymphoblastoid B-cells .
	manualset3
116700	3	404566	5	NULL	NULL	0	NULL	placental serum	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A factor was discovered in the human serum , placental serum from the umbilical cord of pregnant women and sera of peripheral blood from some healthy donors , which induces one of the late stages of differentiation : switching of IgM to IgG synthesis in the RPMI-6410t line of human lymphoblastoid B-cells .
	manualset3
116701	4	404566	5	NULL	NULL	0	NULL	umbilical cord 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A factor was discovered in the human serum , placental serum from the umbilical cord of pregnant women and sera of peripheral blood from some healthy donors , which induces one of the late stages of differentiation : switching of IgM to IgG synthesis in the RPMI-6410t line of human lymphoblastoid B-cells .
	manualset3
116702	5	404566	5	NULL	NULL	0	NULL	pregnant women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A factor was discovered in the human serum , placental serum from the umbilical cord of pregnant women and sera of peripheral blood from some healthy donors , which induces one of the late stages of differentiation : switching of IgM to IgG synthesis in the RPMI-6410t line of human lymphoblastoid B-cells .
	manualset3
116703	6	404566	5	NULL	NULL	0	NULL	sera 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A factor was discovered in the human serum , placental serum from the umbilical cord of pregnant women and sera of peripheral blood from some healthy donors , which induces one of the late stages of differentiation : switching of IgM to IgG synthesis in the RPMI-6410t line of human lymphoblastoid B-cells .
	manualset3
116704	7	404566	5	NULL	NULL	0	NULL	peripheral blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	A factor was discovered in the human serum , placental serum from the umbilical cord of pregnant women and sera of peripheral blood from some healthy donors , which induces one of the late stages of differentiation : switching of IgM to IgG synthesis in the RPMI-6410t line of human lymphoblastoid B-cells .
	manualset3
116705	8	404566	5	NULL	NULL	0	NULL	healthy donors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A factor was discovered in the human serum , placental serum from the umbilical cord of pregnant women and sera of peripheral blood from some healthy donors , which induces one of the late stages of differentiation : switching of IgM to IgG synthesis in the RPMI-6410t line of human lymphoblastoid B-cells .
	manualset3
116706	9	404566	5	NULL	NULL	0	NULL	late stages 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A factor was discovered in the human serum , placental serum from the umbilical cord of pregnant women and sera of peripheral blood from some healthy donors , which induces one of the late stages of differentiation : switching of IgM to IgG synthesis in the RPMI-6410t line of human lymphoblastoid B-cells .
	manualset3
116707	10	404566	5	NULL	NULL	0	NULL	differentiation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A factor was discovered in the human serum , placental serum from the umbilical cord of pregnant women and sera of peripheral blood from some healthy donors , which induces one of the late stages of differentiation : switching of IgM to IgG synthesis in the RPMI-6410t line of human lymphoblastoid B-cells .
	manualset3
116708	11	404566	5	NULL	NULL	0	NULL	IgM	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A factor was discovered in the human serum , placental serum from the umbilical cord of pregnant women and sera of peripheral blood from some healthy donors , which induces one of the late stages of differentiation : switching of IgM to IgG synthesis in the RPMI-6410t line of human lymphoblastoid B-cells .
	manualset3
116709	12	404566	5	NULL	NULL	0	NULL	IgG synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A factor was discovered in the human serum , placental serum from the umbilical cord of pregnant women and sera of peripheral blood from some healthy donors , which induces one of the late stages of differentiation : switching of IgM to IgG synthesis in the RPMI-6410t line of human lymphoblastoid B-cells .
	manualset3
116710	13	404566	5	NULL	NULL	0	NULL	RPMI-6410t line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A factor was discovered in the human serum , placental serum from the umbilical cord of pregnant women and sera of peripheral blood from some healthy donors , which induces one of the late stages of differentiation : switching of IgM to IgG synthesis in the RPMI-6410t line of human lymphoblastoid B-cells .
	manualset3
116711	14	404566	5	NULL	NULL	0	NULL	human lymphoblastoid B-cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A factor was discovered in the human serum , placental serum from the umbilical cord of pregnant women and sera of peripheral blood from some healthy donors , which induces one of the late stages of differentiation : switching of IgM to IgG synthesis in the RPMI-6410t line of human lymphoblastoid B-cells .
	manualset3
116712	1	404567	5	NULL	NULL	NULL	NULL	approach 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our approach is based on an unsupervised change detection method that searches for the most dissimilar region ( axis-parallel bounding boxes ) between the left and the right halves of a brain in an axial view MR slice .
	manualset3
116713	2	404567	5	NULL	NULL	NULL	NULL	unsupervised change detection method	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our approach is based on an unsupervised change detection method that searches for the most dissimilar region ( axis-parallel bounding boxes ) between the left and the right halves of a brain in an axial view MR slice .
	manualset3
116714	3	404567	5	NULL	NULL	0	NULL	dissimilar region ( axis-parallel bounding boxes )	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our approach is based on an unsupervised change detection method that searches for the most dissimilar region ( axis-parallel bounding boxes ) between the left and the right halves of a brain in an axial view MR slice .
	manualset3
116715	4	404567	5	NULL	NULL	0	NULL	left half	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our approach is based on an unsupervised change detection method that searches for the most dissimilar region ( axis-parallel bounding boxes ) between the left and the right halves of a brain in an axial view MR slice .
	manualset3
116716	5	404567	5	NULL	NULL	0	NULL	right half	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our approach is based on an unsupervised change detection method that searches for the most dissimilar region ( axis-parallel bounding boxes ) between the left and the right halves of a brain in an axial view MR slice .
	manualset3
116717	6	404567	5	NULL	NULL	0	NULL	brain 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our approach is based on an unsupervised change detection method that searches for the most dissimilar region ( axis-parallel bounding boxes ) between the left and the right halves of a brain in an axial view MR slice .
	manualset3
116718	7	404567	5	NULL	NULL	0	NULL	axial view MR slice	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our approach is based on an unsupervised change detection method that searches for the most dissimilar region ( axis-parallel bounding boxes ) between the left and the right halves of a brain in an axial view MR slice .
	manualset3
116719	1	404568	5	NULL	NULL	0	NULL	architectural model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Our architectural model reveals how dimeric AKAP79 concentrates pockets of second messenger responsive enzyme activities at the plasma membrane .
	manualset3
116720	2	404568	5	NULL	NULL	0	NULL	dimeric AKAP79	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our architectural model reveals how dimeric AKAP79 concentrates pockets of second messenger responsive enzyme activities at the plasma membrane .
	manualset3
116721	3	404568	5	NULL	NULL	0	NULL	pockets 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our architectural model reveals how dimeric AKAP79 concentrates pockets of second messenger responsive enzyme activities at the plasma membrane .
	manualset3
116722	4	404568	5	NULL	NULL	0	NULL	second messenger responsive enzyme activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our architectural model reveals how dimeric AKAP79 concentrates pockets of second messenger responsive enzyme activities at the plasma membrane .
	manualset3
116723	5	404568	5	NULL	NULL	0	NULL	plasma membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Our architectural model reveals how dimeric AKAP79 concentrates pockets of second messenger responsive enzyme activities at the plasma membrane .
	manualset3
116724	1	404569	5	NULL	NULL	0	NULL	calibrated measurements	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our calibrated measurements increase 2.5-3-fold protein copy numbers at eukaryotic kinetochores based on previous ratio measurements assuming two Cse4s per budding yeast kinetochore .
	manualset3
116725	2	404569	5	NULL	NULL	0	NULL	2.5-3-fold 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our calibrated measurements increase 2.5-3-fold protein copy numbers at eukaryotic kinetochores based on previous ratio measurements assuming two Cse4s per budding yeast kinetochore .
	manualset3
116726	3	404569	5	NULL	NULL	0	NULL	protein copy numbers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our calibrated measurements increase 2.5-3-fold protein copy numbers at eukaryotic kinetochores based on previous ratio measurements assuming two Cse4s per budding yeast kinetochore .
	manualset3
116727	4	404569	5	NULL	NULL	0	NULL	eukaryotic kinetochores 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Our calibrated measurements increase 2.5-3-fold protein copy numbers at eukaryotic kinetochores based on previous ratio measurements assuming two Cse4s per budding yeast kinetochore .
	manualset3
116728	5	404569	5	NULL	NULL	0	NULL	ratio measurements	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our calibrated measurements increase 2.5-3-fold protein copy numbers at eukaryotic kinetochores based on previous ratio measurements assuming two Cse4s per budding yeast kinetochore .
	manualset3
116729	6	404569	5	NULL	NULL	0	NULL	two Cse4s	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our calibrated measurements increase 2.5-3-fold protein copy numbers at eukaryotic kinetochores based on previous ratio measurements assuming two Cse4s per budding yeast kinetochore .
	manualset3
116730	7	404569	5	NULL	NULL	0	NULL	budding yeast kinetochore	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Our calibrated measurements increase 2.5-3-fold protein copy numbers at eukaryotic kinetochores based on previous ratio measurements assuming two Cse4s per budding yeast kinetochore .
	manualset3
116731	1	404570	5	NULL	NULL	0	NULL	case report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our case report suggests that not only antiviral treatment for HSV , but also anti-inflammatory treatment including steroid and cyclosporine should be considered from the early phase of neonatal systemic HSV infection .
	manualset3
116732	2	404570	5	NULL	NULL	0	NULL	antiviral treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our case report suggests that not only antiviral treatment for HSV , but also anti-inflammatory treatment including steroid and cyclosporine should be considered from the early phase of neonatal systemic HSV infection .
	manualset3
116733	3	404570	5	NULL	NULL	0	NULL	HSV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our case report suggests that not only antiviral treatment for HSV , but also anti-inflammatory treatment including steroid and cyclosporine should be considered from the early phase of neonatal systemic HSV infection .
	manualset3
116734	4	404570	5	NULL	NULL	0	NULL	anti-inflammatory treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our case report suggests that not only antiviral treatment for HSV , but also anti-inflammatory treatment including steroid and cyclosporine should be considered from the early phase of neonatal systemic HSV infection .
	manualset3
116735	5	404570	5	NULL	NULL	0	NULL	steroid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our case report suggests that not only antiviral treatment for HSV , but also anti-inflammatory treatment including steroid and cyclosporine should be considered from the early phase of neonatal systemic HSV infection .
	manualset3
116736	6	404570	5	NULL	NULL	0	NULL	cyclosporine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Our case report suggests that not only antiviral treatment for HSV , but also anti-inflammatory treatment including steroid and cyclosporine should be considered from the early phase of neonatal systemic HSV infection .
	manualset3
116737	7	404570	5	NULL	NULL	0	NULL	early phase 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Our case report suggests that not only antiviral treatment for HSV , but also anti-inflammatory treatment including steroid and cyclosporine should be considered from the early phase of neonatal systemic HSV infection .
	manualset3
116738	8	404570	5	NULL	NULL	0	NULL	neonatal systemic HSV infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our case report suggests that not only antiviral treatment for HSV , but also anti-inflammatory treatment including steroid and cyclosporine should be considered from the early phase of neonatal systemic HSV infection .
	manualset3
116739	1	404571	5	NULL	NULL	0	NULL	computer program BB RADABA 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Our computer program BB RADABA permits the management of breeding and experimental data as well as planning of experiments and evaluation of experimental results .
	manualset3
116740	2	404571	5	NULL	NULL	0	NULL	management 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our computer program BB RADABA permits the management of breeding and experimental data as well as planning of experiments and evaluation of experimental results .
	manualset3
116741	3	404571	5	NULL	NULL	0	NULL	breeding data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our computer program BB RADABA permits the management of breeding and experimental data as well as planning of experiments and evaluation of experimental results .
	manualset3
116742	4	404571	5	NULL	NULL	0	NULL	experimental data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our computer program BB RADABA permits the management of breeding and experimental data as well as planning of experiments and evaluation of experimental results .
	manualset3
116743	5	404571	5	NULL	NULL	0	NULL	experiments 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our computer program BB RADABA permits the management of breeding and experimental data as well as planning of experiments and evaluation of experimental results .
	manualset3
116744	6	404571	5	NULL	NULL	0	NULL	evaluation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our computer program BB RADABA permits the management of breeding and experimental data as well as planning of experiments and evaluation of experimental results .
	manualset3
116745	7	404571	5	NULL	NULL	0	NULL	experimental results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our computer program BB RADABA permits the management of breeding and experimental data as well as planning of experiments and evaluation of experimental results .
	manualset3
116746	1	404572	5	NULL	NULL	0	NULL	understanding 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our current understanding is that ERalpha , not ERbeta is responsible for mediating the effects of estrogens in `` classic '' model systems such as the reproductive tract and skeleton .
	manualset3
116747	2	404572	5	NULL	NULL	0	NULL	ERalpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our current understanding is that ERalpha , not ERbeta is responsible for mediating the effects of estrogens in `` classic '' model systems such as the reproductive tract and skeleton .
	manualset3
116748	3	404572	5	NULL	NULL	0	NULL	ERbeta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our current understanding is that ERalpha , not ERbeta is responsible for mediating the effects of estrogens in `` classic '' model systems such as the reproductive tract and skeleton .
	manualset3
116749	4	404572	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our current understanding is that ERalpha , not ERbeta is responsible for mediating the effects of estrogens in `` classic '' model systems such as the reproductive tract and skeleton .
	manualset3
116750	5	404572	5	NULL	NULL	0	NULL	estrogens 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Our current understanding is that ERalpha , not ERbeta is responsible for mediating the effects of estrogens in `` classic '' model systems such as the reproductive tract and skeleton .
	manualset3
116751	6	404572	5	NULL	NULL	0	NULL	model systems 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our current understanding is that ERalpha , not ERbeta is responsible for mediating the effects of estrogens in `` classic '' model systems such as the reproductive tract and skeleton .
	manualset3
116752	7	404572	5	NULL	NULL	0	NULL	reproductive tract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our current understanding is that ERalpha , not ERbeta is responsible for mediating the effects of estrogens in `` classic '' model systems such as the reproductive tract and skeleton .
	manualset3
116753	8	404572	5	NULL	NULL	0	NULL	skeleton 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our current understanding is that ERalpha , not ERbeta is responsible for mediating the effects of estrogens in `` classic '' model systems such as the reproductive tract and skeleton .
	manualset3
116754	1	404573	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data further suggested that these associations may be best understood in terms of interactions between various processing biases alluded in the most recent cognitive accounts of schizophrenia symptoms .
	manualset3
116755	2	404573	5	NULL	NULL	0	NULL	associations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data further suggested that these associations may be best understood in terms of interactions between various processing biases alluded in the most recent cognitive accounts of schizophrenia symptoms .
	manualset3
116756	3	404573	5	NULL	NULL	0	NULL	interactions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data further suggested that these associations may be best understood in terms of interactions between various processing biases alluded in the most recent cognitive accounts of schizophrenia symptoms .
	manualset3
116757	4	404573	5	NULL	NULL	0	NULL	cognitive accounts	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data further suggested that these associations may be best understood in terms of interactions between various processing biases alluded in the most recent cognitive accounts of schizophrenia symptoms .
	manualset3
116758	5	404573	5	NULL	NULL	0	NULL	schizophrenia symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data further suggested that these associations may be best understood in terms of interactions between various processing biases alluded in the most recent cognitive accounts of schizophrenia symptoms .
	manualset3
121229	6	404573	5	NULL	NULL	0	NULL	processing biases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data further suggested that these associations may be best understood in terms of interactions between various processing biases alluded in the most recent cognitive accounts of schizophrenia symptoms .
	manualset3
116759	1	404574	5	NULL	NULL	0	NULL	family 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A family is described in which three siblings had congenital abnormalities consistent with partial trisomy 9q syndrome .
	manualset3
116760	2	404574	5	NULL	NULL	0	NULL	three 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A family is described in which three siblings had congenital abnormalities consistent with partial trisomy 9q syndrome .
	manualset3
116761	3	404574	5	NULL	NULL	0	NULL	siblings 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A family is described in which three siblings had congenital abnormalities consistent with partial trisomy 9q syndrome .
	manualset3
116762	4	404574	5	NULL	NULL	0	NULL	congenital abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A family is described in which three siblings had congenital abnormalities consistent with partial trisomy 9q syndrome .
	manualset3
116763	5	404574	5	NULL	NULL	0	NULL	partial trisomy 9q syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A family is described in which three siblings had congenital abnormalities consistent with partial trisomy 9q syndrome .
	manualset3
116764	1	404575	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data further suggest that some of the pathologies seen in AT could arise as a consequence of an inability to respond normally to oxidative damage .
	manualset3
116765	2	404575	5	NULL	NULL	0	NULL	pathologies 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data further suggest that some of the pathologies seen in AT could arise as a consequence of an inability to respond normally to oxidative damage .
	manualset3
116766	3	404575	5	NULL	NULL	0	NULL	AT	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data further suggest that some of the pathologies seen in AT could arise as a consequence of an inability to respond normally to oxidative damage .
	manualset3
116767	4	404575	5	NULL	NULL	0	NULL	consequence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data further suggest that some of the pathologies seen in AT could arise as a consequence of an inability to respond normally to oxidative damage .
	manualset3
116768	5	404575	5	NULL	NULL	NULL	NULL	inability to respond 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our data further suggest that some of the pathologies seen in AT could arise as a consequence of an inability to respond normally to oxidative damage .
	manualset3
116769	6	404575	5	NULL	NULL	0	NULL	oxidative damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data further suggest that some of the pathologies seen in AT could arise as a consequence of an inability to respond normally to oxidative damage .
	manualset3
116770	1	404576	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data strongly suggest that GHRH plays a crucial role in the development of EAE and may provide the basis for a novel therapeutic approach protecting from autoimmune diseases .
	manualset3
116771	2	404576	5	NULL	NULL	0	NULL	GHRH 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data strongly suggest that GHRH plays a crucial role in the development of EAE and may provide the basis for a novel therapeutic approach protecting from autoimmune diseases .
	manualset3
116772	3	404576	5	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data strongly suggest that GHRH plays a crucial role in the development of EAE and may provide the basis for a novel therapeutic approach protecting from autoimmune diseases .
	manualset3
116773	4	404576	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data strongly suggest that GHRH plays a crucial role in the development of EAE and may provide the basis for a novel therapeutic approach protecting from autoimmune diseases .
	manualset3
116774	5	404576	5	NULL	NULL	0	NULL	EAE 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data strongly suggest that GHRH plays a crucial role in the development of EAE and may provide the basis for a novel therapeutic approach protecting from autoimmune diseases .
	manualset3
116775	6	404576	5	NULL	NULL	0	NULL	novel therapeutic approach	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data strongly suggest that GHRH plays a crucial role in the development of EAE and may provide the basis for a novel therapeutic approach protecting from autoimmune diseases .
	manualset3
116776	7	404576	5	NULL	NULL	0	NULL	autoimmune diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our data strongly suggest that GHRH plays a crucial role in the development of EAE and may provide the basis for a novel therapeutic approach protecting from autoimmune diseases .
	manualset3
116777	1	404577	5	NULL	NULL	0	NULL	density functional theory ( DFT )	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Our density functional theory ( DFT ) , time-dependent DFT ( TDDFT ) , and complete active space self-consistent field ( CASSCF ) calculations indicate that the double-proton-transfer process in the ground and first singlet pi -- ) pi * excited state in BP ( OH ) ( NH ( 2 ) ) presents features that are between those of their `` parents '' .
	manualset3
116778	2	404577	5	NULL	NULL	0	NULL	time-dependent DFT ( TDDFT )	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Our density functional theory ( DFT ) , time-dependent DFT ( TDDFT ) , and complete active space self-consistent field ( CASSCF ) calculations indicate that the double-proton-transfer process in the ground and first singlet pi -- ) pi * excited state in BP ( OH ) ( NH ( 2 ) ) presents features that are between those of their `` parents '' .
	manualset3
116779	3	404577	5	NULL	NULL	0	NULL	complete active space self-consistent field ( CASSCF ) calculations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our density functional theory ( DFT ) , time-dependent DFT ( TDDFT ) , and complete active space self-consistent field ( CASSCF ) calculations indicate that the double-proton-transfer process in the ground and first singlet pi -- ) pi * excited state in BP ( OH ) ( NH ( 2 ) ) presents features that are between those of their `` parents '' .
	manualset3
116780	4	404577	5	NULL	NULL	0	NULL	double-proton-transfer process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our density functional theory ( DFT ) , time-dependent DFT ( TDDFT ) , and complete active space self-consistent field ( CASSCF ) calculations indicate that the double-proton-transfer process in the ground and first singlet pi -- ) pi * excited state in BP ( OH ) ( NH ( 2 ) ) presents features that are between those of their `` parents '' .
	manualset3
116781	5	404577	5	NULL	NULL	0	NULL	 ground and first singlet pi -- ) pi * excited state	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our density functional theory ( DFT ) , time-dependent DFT ( TDDFT ) , and complete active space self-consistent field ( CASSCF ) calculations indicate that the double-proton-transfer process in the ground and first singlet pi -- ) pi * excited state in BP ( OH ) ( NH ( 2 ) ) presents features that are between those of their `` parents '' .
	manualset3
116782	6	404577	5	NULL	NULL	0	NULL	BP ( OH ) ( NH ( 2 ) ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our density functional theory ( DFT ) , time-dependent DFT ( TDDFT ) , and complete active space self-consistent field ( CASSCF ) calculations indicate that the double-proton-transfer process in the ground and first singlet pi -- ) pi * excited state in BP ( OH ) ( NH ( 2 ) ) presents features that are between those of their `` parents '' .
	manualset3
116783	7	404577	5	NULL	NULL	NULL	NULL	parents 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our density functional theory ( DFT ) , time-dependent DFT ( TDDFT ) , and complete active space self-consistent field ( CASSCF ) calculations indicate that the double-proton-transfer process in the ground and first singlet pi -- ) pi * excited state in BP ( OH ) ( NH ( 2 ) ) presents features that are between those of their `` parents '' .
	manualset3
116784	1	404578	5	NULL	NULL	0	NULL	epidemiologic survey	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our epidemiologic survey confirms the rareness of perinatal pneumococcal infection and the ability of these organisms to cause morbidity in both mothers and infants .
	manualset3
116785	2	404578	5	NULL	NULL	0	NULL	perinatal pneumococcal infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our epidemiologic survey confirms the rareness of perinatal pneumococcal infection and the ability of these organisms to cause morbidity in both mothers and infants .
	manualset3
116786	3	404578	5	NULL	NULL	0	NULL	ability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our epidemiologic survey confirms the rareness of perinatal pneumococcal infection and the ability of these organisms to cause morbidity in both mothers and infants .
	manualset3
116787	4	404578	5	NULL	NULL	0	NULL	organisms 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our epidemiologic survey confirms the rareness of perinatal pneumococcal infection and the ability of these organisms to cause morbidity in both mothers and infants .
	manualset3
116788	5	404578	5	NULL	NULL	0	NULL	morbidity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our epidemiologic survey confirms the rareness of perinatal pneumococcal infection and the ability of these organisms to cause morbidity in both mothers and infants .
	manualset3
116789	6	404578	5	NULL	NULL	0	NULL	mothers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our epidemiologic survey confirms the rareness of perinatal pneumococcal infection and the ability of these organisms to cause morbidity in both mothers and infants .
	manualset3
116790	7	404578	5	NULL	NULL	0	NULL	infants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our epidemiologic survey confirms the rareness of perinatal pneumococcal infection and the ability of these organisms to cause morbidity in both mothers and infants .
	manualset3
116791	1	404579	5	NULL	NULL	0	NULL	experience 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experience covers the surgical treatment of 200 patients with scars due to fire , acids , and land mines .
	manualset3
116792	2	404579	5	NULL	NULL	0	NULL	surgical treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experience covers the surgical treatment of 200 patients with scars due to fire , acids , and land mines .
	manualset3
116793	3	404579	5	NULL	NULL	0	NULL	200 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experience covers the surgical treatment of 200 patients with scars due to fire , acids , and land mines .
	manualset3
116794	4	404579	5	NULL	NULL	0	NULL	scars 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experience covers the surgical treatment of 200 patients with scars due to fire , acids , and land mines .
	manualset3
116795	5	404579	5	NULL	NULL	0	NULL	fire 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experience covers the surgical treatment of 200 patients with scars due to fire , acids , and land mines .
	manualset3
116796	6	404579	5	NULL	NULL	0	NULL	acids 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experience covers the surgical treatment of 200 patients with scars due to fire , acids , and land mines .
	manualset3
116797	7	404579	5	NULL	NULL	0	NULL	land mines	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experience covers the surgical treatment of 200 patients with scars due to fire , acids , and land mines .
	manualset3
116798	1	404580	5	NULL	NULL	0	NULL	experience 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experience in thymic hyperplasia using 67Ga-citrate , 111In-pentetreotide and 201Tl-chloride .
	manualset3
116799	2	404580	5	NULL	NULL	0	NULL	thymic hyperplasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experience in thymic hyperplasia using 67Ga-citrate , 111In-pentetreotide and 201Tl-chloride .
	manualset3
116800	3	404580	5	NULL	NULL	NULL	NULL	67Ga-citrate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our experience in thymic hyperplasia using 67Ga-citrate , 111In-pentetreotide and 201Tl-chloride .
	manualset3
116801	4	404580	5	NULL	NULL	0	NULL	111In-pentetreotide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experience in thymic hyperplasia using 67Ga-citrate , 111In-pentetreotide and 201Tl-chloride .
	manualset3
116802	5	404580	5	NULL	NULL	0	NULL	201Tl-chloride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experience in thymic hyperplasia using 67Ga-citrate , 111In-pentetreotide and 201Tl-chloride .
	manualset3
116855	1	404581	5	NULL	NULL	0	NULL	experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experience suggests that the decrease of immunosuppressive drug therapy , followed by the nephrectomy of the transplanted kidney if signs of rejection are present , and right hemicolectomy are the best therapy .
	manualset3
116856	2	404581	5	NULL	NULL	0	NULL	immunosuppressive drug therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experience suggests that the decrease of immunosuppressive drug therapy , followed by the nephrectomy of the transplanted kidney if signs of rejection are present , and right hemicolectomy are the best therapy .
	manualset3
116857	3	404581	5	NULL	NULL	0	NULL	nephrectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experience suggests that the decrease of immunosuppressive drug therapy , followed by the nephrectomy of the transplanted kidney if signs of rejection are present , and right hemicolectomy are the best therapy .
	manualset3
116858	4	404581	5	NULL	NULL	0	NULL	transplanted kidney	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experience suggests that the decrease of immunosuppressive drug therapy , followed by the nephrectomy of the transplanted kidney if signs of rejection are present , and right hemicolectomy are the best therapy .
	manualset3
116859	5	404581	5	NULL	NULL	0	NULL	signs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experience suggests that the decrease of immunosuppressive drug therapy , followed by the nephrectomy of the transplanted kidney if signs of rejection are present , and right hemicolectomy are the best therapy .
	manualset3
116860	6	404581	5	NULL	NULL	0	NULL	rejection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experience suggests that the decrease of immunosuppressive drug therapy , followed by the nephrectomy of the transplanted kidney if signs of rejection are present , and right hemicolectomy are the best therapy .
	manualset3
116861	7	404581	5	NULL	NULL	0	NULL	hemicolectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experience suggests that the decrease of immunosuppressive drug therapy , followed by the nephrectomy of the transplanted kidney if signs of rejection are present , and right hemicolectomy are the best therapy .
	manualset3
116862	8	404581	5	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experience suggests that the decrease of immunosuppressive drug therapy , followed by the nephrectomy of the transplanted kidney if signs of rejection are present , and right hemicolectomy are the best therapy .
	manualset3
121230	9	404581	5	NULL	NULL	0	NULL	decrease 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experience suggests that the decrease of immunosuppressive drug therapy , followed by the nephrectomy of the transplanted kidney if signs of rejection are present , and right hemicolectomy are the best therapy .
	manualset3
116863	1	404582	5	NULL	NULL	0	NULL	experiment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experiment further demonstrated that , in vitro , ( 1 ) CASE inhibits TGF-beta ( 1 ) - dependent Smad2 phosphorylation at C-terminal region and Smad2 and Smad3 phosphorylation at linker region in MFBs in a dose-dependent manner ; ( 2 ) CASE decreases the level of Smad 2/3/4 complex in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; ( 3 ) CASE inhibits PAI-1 transcriptional activity in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; and ( 4 ) CASE markedly decreases c-Jun N-terminal kinase ( JNK ) phosphorylation in MFBs induced by TGF-beta ( 1 ) .
	manualset3
116864	2	404582	5	NULL	NULL	0	NULL	CASE	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experiment further demonstrated that , in vitro , ( 1 ) CASE inhibits TGF-beta ( 1 ) - dependent Smad2 phosphorylation at C-terminal region and Smad2 and Smad3 phosphorylation at linker region in MFBs in a dose-dependent manner ; ( 2 ) CASE decreases the level of Smad 2/3/4 complex in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; ( 3 ) CASE inhibits PAI-1 transcriptional activity in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; and ( 4 ) CASE markedly decreases c-Jun N-terminal kinase ( JNK ) phosphorylation in MFBs induced by TGF-beta ( 1 ) .
	manualset3
116865	3	404582	5	NULL	NULL	0	NULL	TGF-beta ( 1 ) - dependent Smad2 phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experiment further demonstrated that , in vitro , ( 1 ) CASE inhibits TGF-beta ( 1 ) - dependent Smad2 phosphorylation at C-terminal region and Smad2 and Smad3 phosphorylation at linker region in MFBs in a dose-dependent manner ; ( 2 ) CASE decreases the level of Smad 2/3/4 complex in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; ( 3 ) CASE inhibits PAI-1 transcriptional activity in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; and ( 4 ) CASE markedly decreases c-Jun N-terminal kinase ( JNK ) phosphorylation in MFBs induced by TGF-beta ( 1 ) .
	manualset3
116866	4	404582	5	NULL	NULL	0	NULL	C-terminal region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experiment further demonstrated that , in vitro , ( 1 ) CASE inhibits TGF-beta ( 1 ) - dependent Smad2 phosphorylation at C-terminal region and Smad2 and Smad3 phosphorylation at linker region in MFBs in a dose-dependent manner ; ( 2 ) CASE decreases the level of Smad 2/3/4 complex in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; ( 3 ) CASE inhibits PAI-1 transcriptional activity in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; and ( 4 ) CASE markedly decreases c-Jun N-terminal kinase ( JNK ) phosphorylation in MFBs induced by TGF-beta ( 1 ) .
	manualset3
116867	5	404582	5	NULL	NULL	0	NULL	Smad2 phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experiment further demonstrated that , in vitro , ( 1 ) CASE inhibits TGF-beta ( 1 ) - dependent Smad2 phosphorylation at C-terminal region and Smad2 and Smad3 phosphorylation at linker region in MFBs in a dose-dependent manner ; ( 2 ) CASE decreases the level of Smad 2/3/4 complex in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; ( 3 ) CASE inhibits PAI-1 transcriptional activity in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; and ( 4 ) CASE markedly decreases c-Jun N-terminal kinase ( JNK ) phosphorylation in MFBs induced by TGF-beta ( 1 ) .
	manualset3
116868	6	404582	5	NULL	NULL	0	NULL	Smad3 phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experiment further demonstrated that , in vitro , ( 1 ) CASE inhibits TGF-beta ( 1 ) - dependent Smad2 phosphorylation at C-terminal region and Smad2 and Smad3 phosphorylation at linker region in MFBs in a dose-dependent manner ; ( 2 ) CASE decreases the level of Smad 2/3/4 complex in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; ( 3 ) CASE inhibits PAI-1 transcriptional activity in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; and ( 4 ) CASE markedly decreases c-Jun N-terminal kinase ( JNK ) phosphorylation in MFBs induced by TGF-beta ( 1 ) .
	manualset3
116869	7	404582	5	NULL	NULL	0	NULL	linker region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experiment further demonstrated that , in vitro , ( 1 ) CASE inhibits TGF-beta ( 1 ) - dependent Smad2 phosphorylation at C-terminal region and Smad2 and Smad3 phosphorylation at linker region in MFBs in a dose-dependent manner ; ( 2 ) CASE decreases the level of Smad 2/3/4 complex in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; ( 3 ) CASE inhibits PAI-1 transcriptional activity in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; and ( 4 ) CASE markedly decreases c-Jun N-terminal kinase ( JNK ) phosphorylation in MFBs induced by TGF-beta ( 1 ) .
	manualset3
116870	8	404582	5	NULL	NULL	0	NULL	MFBs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experiment further demonstrated that , in vitro , ( 1 ) CASE inhibits TGF-beta ( 1 ) - dependent Smad2 phosphorylation at C-terminal region and Smad2 and Smad3 phosphorylation at linker region in MFBs in a dose-dependent manner ; ( 2 ) CASE decreases the level of Smad 2/3/4 complex in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; ( 3 ) CASE inhibits PAI-1 transcriptional activity in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; and ( 4 ) CASE markedly decreases c-Jun N-terminal kinase ( JNK ) phosphorylation in MFBs induced by TGF-beta ( 1 ) .
	manualset3
116871	9	404582	5	NULL	NULL	0	NULL	dose-dependent manner	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experiment further demonstrated that , in vitro , ( 1 ) CASE inhibits TGF-beta ( 1 ) - dependent Smad2 phosphorylation at C-terminal region and Smad2 and Smad3 phosphorylation at linker region in MFBs in a dose-dependent manner ; ( 2 ) CASE decreases the level of Smad 2/3/4 complex in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; ( 3 ) CASE inhibits PAI-1 transcriptional activity in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; and ( 4 ) CASE markedly decreases c-Jun N-terminal kinase ( JNK ) phosphorylation in MFBs induced by TGF-beta ( 1 ) .
	manualset3
116873	11	404582	5	NULL	NULL	0	NULL	level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experiment further demonstrated that , in vitro , ( 1 ) CASE inhibits TGF-beta ( 1 ) - dependent Smad2 phosphorylation at C-terminal region and Smad2 and Smad3 phosphorylation at linker region in MFBs in a dose-dependent manner ; ( 2 ) CASE decreases the level of Smad 2/3/4 complex in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; ( 3 ) CASE inhibits PAI-1 transcriptional activity in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; and ( 4 ) CASE markedly decreases c-Jun N-terminal kinase ( JNK ) phosphorylation in MFBs induced by TGF-beta ( 1 ) .
	manualset3
116874	12	404582	5	NULL	NULL	0	NULL	Smad 2/3/4 complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experiment further demonstrated that , in vitro , ( 1 ) CASE inhibits TGF-beta ( 1 ) - dependent Smad2 phosphorylation at C-terminal region and Smad2 and Smad3 phosphorylation at linker region in MFBs in a dose-dependent manner ; ( 2 ) CASE decreases the level of Smad 2/3/4 complex in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; ( 3 ) CASE inhibits PAI-1 transcriptional activity in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; and ( 4 ) CASE markedly decreases c-Jun N-terminal kinase ( JNK ) phosphorylation in MFBs induced by TGF-beta ( 1 ) .
	manualset3
116875	13	404582	5	NULL	NULL	0	NULL	MFBs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experiment further demonstrated that , in vitro , ( 1 ) CASE inhibits TGF-beta ( 1 ) - dependent Smad2 phosphorylation at C-terminal region and Smad2 and Smad3 phosphorylation at linker region in MFBs in a dose-dependent manner ; ( 2 ) CASE decreases the level of Smad 2/3/4 complex in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; ( 3 ) CASE inhibits PAI-1 transcriptional activity in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; and ( 4 ) CASE markedly decreases c-Jun N-terminal kinase ( JNK ) phosphorylation in MFBs induced by TGF-beta ( 1 ) .
	manualset3
116876	14	404582	5	NULL	NULL	0	NULL	TGF-beta ( 1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experiment further demonstrated that , in vitro , ( 1 ) CASE inhibits TGF-beta ( 1 ) - dependent Smad2 phosphorylation at C-terminal region and Smad2 and Smad3 phosphorylation at linker region in MFBs in a dose-dependent manner ; ( 2 ) CASE decreases the level of Smad 2/3/4 complex in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; ( 3 ) CASE inhibits PAI-1 transcriptional activity in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; and ( 4 ) CASE markedly decreases c-Jun N-terminal kinase ( JNK ) phosphorylation in MFBs induced by TGF-beta ( 1 ) .
	manualset3
116877	15	404582	5	NULL	NULL	0	NULL	dose-dependent manner	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experiment further demonstrated that , in vitro , ( 1 ) CASE inhibits TGF-beta ( 1 ) - dependent Smad2 phosphorylation at C-terminal region and Smad2 and Smad3 phosphorylation at linker region in MFBs in a dose-dependent manner ; ( 2 ) CASE decreases the level of Smad 2/3/4 complex in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; ( 3 ) CASE inhibits PAI-1 transcriptional activity in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; and ( 4 ) CASE markedly decreases c-Jun N-terminal kinase ( JNK ) phosphorylation in MFBs induced by TGF-beta ( 1 ) .
	manualset3
116878	16	404582	5	NULL	NULL	0	NULL	CASE	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experiment further demonstrated that , in vitro , ( 1 ) CASE inhibits TGF-beta ( 1 ) - dependent Smad2 phosphorylation at C-terminal region and Smad2 and Smad3 phosphorylation at linker region in MFBs in a dose-dependent manner ; ( 2 ) CASE decreases the level of Smad 2/3/4 complex in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; ( 3 ) CASE inhibits PAI-1 transcriptional activity in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; and ( 4 ) CASE markedly decreases c-Jun N-terminal kinase ( JNK ) phosphorylation in MFBs induced by TGF-beta ( 1 ) .
	manualset3
116879	17	404582	5	NULL	NULL	0	NULL	PAI-1 transcriptional activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experiment further demonstrated that , in vitro , ( 1 ) CASE inhibits TGF-beta ( 1 ) - dependent Smad2 phosphorylation at C-terminal region and Smad2 and Smad3 phosphorylation at linker region in MFBs in a dose-dependent manner ; ( 2 ) CASE decreases the level of Smad 2/3/4 complex in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; ( 3 ) CASE inhibits PAI-1 transcriptional activity in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; and ( 4 ) CASE markedly decreases c-Jun N-terminal kinase ( JNK ) phosphorylation in MFBs induced by TGF-beta ( 1 ) .
	manualset3
116880	18	404582	5	NULL	NULL	0	NULL	MFBs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experiment further demonstrated that , in vitro , ( 1 ) CASE inhibits TGF-beta ( 1 ) - dependent Smad2 phosphorylation at C-terminal region and Smad2 and Smad3 phosphorylation at linker region in MFBs in a dose-dependent manner ; ( 2 ) CASE decreases the level of Smad 2/3/4 complex in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; ( 3 ) CASE inhibits PAI-1 transcriptional activity in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; and ( 4 ) CASE markedly decreases c-Jun N-terminal kinase ( JNK ) phosphorylation in MFBs induced by TGF-beta ( 1 ) .
	manualset3
116881	19	404582	5	NULL	NULL	0	NULL	TGF-beta ( 1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experiment further demonstrated that , in vitro , ( 1 ) CASE inhibits TGF-beta ( 1 ) - dependent Smad2 phosphorylation at C-terminal region and Smad2 and Smad3 phosphorylation at linker region in MFBs in a dose-dependent manner ; ( 2 ) CASE decreases the level of Smad 2/3/4 complex in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; ( 3 ) CASE inhibits PAI-1 transcriptional activity in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; and ( 4 ) CASE markedly decreases c-Jun N-terminal kinase ( JNK ) phosphorylation in MFBs induced by TGF-beta ( 1 ) .
	manualset3
116882	20	404582	5	NULL	NULL	0	NULL	dose-dependent manner 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experiment further demonstrated that , in vitro , ( 1 ) CASE inhibits TGF-beta ( 1 ) - dependent Smad2 phosphorylation at C-terminal region and Smad2 and Smad3 phosphorylation at linker region in MFBs in a dose-dependent manner ; ( 2 ) CASE decreases the level of Smad 2/3/4 complex in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; ( 3 ) CASE inhibits PAI-1 transcriptional activity in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; and ( 4 ) CASE markedly decreases c-Jun N-terminal kinase ( JNK ) phosphorylation in MFBs induced by TGF-beta ( 1 ) .
	manualset3
116883	21	404582	5	NULL	NULL	0	NULL	CASE	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experiment further demonstrated that , in vitro , ( 1 ) CASE inhibits TGF-beta ( 1 ) - dependent Smad2 phosphorylation at C-terminal region and Smad2 and Smad3 phosphorylation at linker region in MFBs in a dose-dependent manner ; ( 2 ) CASE decreases the level of Smad 2/3/4 complex in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; ( 3 ) CASE inhibits PAI-1 transcriptional activity in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; and ( 4 ) CASE markedly decreases c-Jun N-terminal kinase ( JNK ) phosphorylation in MFBs induced by TGF-beta ( 1 ) .
	manualset3
116884	22	404582	5	NULL	NULL	0	NULL	c-Jun N-terminal kinase ( JNK ) phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experiment further demonstrated that , in vitro , ( 1 ) CASE inhibits TGF-beta ( 1 ) - dependent Smad2 phosphorylation at C-terminal region and Smad2 and Smad3 phosphorylation at linker region in MFBs in a dose-dependent manner ; ( 2 ) CASE decreases the level of Smad 2/3/4 complex in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; ( 3 ) CASE inhibits PAI-1 transcriptional activity in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; and ( 4 ) CASE markedly decreases c-Jun N-terminal kinase ( JNK ) phosphorylation in MFBs induced by TGF-beta ( 1 ) .
	manualset3
116885	23	404582	5	NULL	NULL	0	NULL	MFBs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experiment further demonstrated that , in vitro , ( 1 ) CASE inhibits TGF-beta ( 1 ) - dependent Smad2 phosphorylation at C-terminal region and Smad2 and Smad3 phosphorylation at linker region in MFBs in a dose-dependent manner ; ( 2 ) CASE decreases the level of Smad 2/3/4 complex in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; ( 3 ) CASE inhibits PAI-1 transcriptional activity in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; and ( 4 ) CASE markedly decreases c-Jun N-terminal kinase ( JNK ) phosphorylation in MFBs induced by TGF-beta ( 1 ) .
	manualset3
116886	24	404582	5	NULL	NULL	0	NULL	TGF-beta ( 1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our experiment further demonstrated that , in vitro , ( 1 ) CASE inhibits TGF-beta ( 1 ) - dependent Smad2 phosphorylation at C-terminal region and Smad2 and Smad3 phosphorylation at linker region in MFBs in a dose-dependent manner ; ( 2 ) CASE decreases the level of Smad 2/3/4 complex in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; ( 3 ) CASE inhibits PAI-1 transcriptional activity in MFBs induced by TGF-beta ( 1 ) in a dose-dependent manner ; and ( 4 ) CASE markedly decreases c-Jun N-terminal kinase ( JNK ) phosphorylation in MFBs induced by TGF-beta ( 1 ) .
	manualset3
116887	1	404583	5	NULL	NULL	0	NULL	family	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A family of developmentally excised DNA elements in Tetrahymena is under selective pressure to maintain an open reading frame encoding an integrase-like protein .
	manualset3
116888	2	404583	5	NULL	NULL	0	NULL	developmentally excised DNA elements	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A family of developmentally excised DNA elements in Tetrahymena is under selective pressure to maintain an open reading frame encoding an integrase-like protein .
	manualset3
116889	3	404583	5	NULL	NULL	0	NULL	Tetrahymena	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A family of developmentally excised DNA elements in Tetrahymena is under selective pressure to maintain an open reading frame encoding an integrase-like protein .
	manualset3
116890	4	404583	5	NULL	NULL	0	NULL	selective pressure 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A family of developmentally excised DNA elements in Tetrahymena is under selective pressure to maintain an open reading frame encoding an integrase-like protein .
	manualset3
116891	5	404583	5	NULL	NULL	0	NULL	open reading frame	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A family of developmentally excised DNA elements in Tetrahymena is under selective pressure to maintain an open reading frame encoding an integrase-like protein .
	manualset3
116892	6	404583	5	NULL	NULL	0	NULL	integrase-like protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A family of developmentally excised DNA elements in Tetrahymena is under selective pressure to maintain an open reading frame encoding an integrase-like protein .
	manualset3
116893	1	404584	5	NULL	NULL	0	NULL	findings 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings on host anti-donor alloresponse , as revealed by skin allograft survival and cytotoxic T lymphocyte assays , indicated that the administration of syngeneic DC presenting K ( bm1 ) donor-derived allopeptides through the indirect pathway of antigen presentation was not sufficient to induce cross-tolerance to alloreactive CD8 ( + ) T cells responding to bm1 alloantigens in a murine model of skin allograft transplantation across an MHC class I mismatched barrier .
	manualset3
116894	2	404584	5	NULL	NULL	0	NULL	host anti-donor alloresponse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings on host anti-donor alloresponse , as revealed by skin allograft survival and cytotoxic T lymphocyte assays , indicated that the administration of syngeneic DC presenting K ( bm1 ) donor-derived allopeptides through the indirect pathway of antigen presentation was not sufficient to induce cross-tolerance to alloreactive CD8 ( + ) T cells responding to bm1 alloantigens in a murine model of skin allograft transplantation across an MHC class I mismatched barrier .
	manualset3
116895	3	404584	5	NULL	NULL	0	NULL	skin allograft survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings on host anti-donor alloresponse , as revealed by skin allograft survival and cytotoxic T lymphocyte assays , indicated that the administration of syngeneic DC presenting K ( bm1 ) donor-derived allopeptides through the indirect pathway of antigen presentation was not sufficient to induce cross-tolerance to alloreactive CD8 ( + ) T cells responding to bm1 alloantigens in a murine model of skin allograft transplantation across an MHC class I mismatched barrier .
	manualset3
116896	4	404584	5	NULL	NULL	0	NULL	cytotoxic T lymphocyte assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings on host anti-donor alloresponse , as revealed by skin allograft survival and cytotoxic T lymphocyte assays , indicated that the administration of syngeneic DC presenting K ( bm1 ) donor-derived allopeptides through the indirect pathway of antigen presentation was not sufficient to induce cross-tolerance to alloreactive CD8 ( + ) T cells responding to bm1 alloantigens in a murine model of skin allograft transplantation across an MHC class I mismatched barrier .
	manualset3
116897	5	404584	5	NULL	NULL	0	NULL	administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings on host anti-donor alloresponse , as revealed by skin allograft survival and cytotoxic T lymphocyte assays , indicated that the administration of syngeneic DC presenting K ( bm1 ) donor-derived allopeptides through the indirect pathway of antigen presentation was not sufficient to induce cross-tolerance to alloreactive CD8 ( + ) T cells responding to bm1 alloantigens in a murine model of skin allograft transplantation across an MHC class I mismatched barrier .
	manualset3
116898	6	404584	5	NULL	NULL	0	NULL	syngeneic DC presenting K ( bm1 ) donor-derived allopeptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings on host anti-donor alloresponse , as revealed by skin allograft survival and cytotoxic T lymphocyte assays , indicated that the administration of syngeneic DC presenting K ( bm1 ) donor-derived allopeptides through the indirect pathway of antigen presentation was not sufficient to induce cross-tolerance to alloreactive CD8 ( + ) T cells responding to bm1 alloantigens in a murine model of skin allograft transplantation across an MHC class I mismatched barrier .
	manualset3
116899	7	404584	5	NULL	NULL	0	NULL	indirect pathway 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings on host anti-donor alloresponse , as revealed by skin allograft survival and cytotoxic T lymphocyte assays , indicated that the administration of syngeneic DC presenting K ( bm1 ) donor-derived allopeptides through the indirect pathway of antigen presentation was not sufficient to induce cross-tolerance to alloreactive CD8 ( + ) T cells responding to bm1 alloantigens in a murine model of skin allograft transplantation across an MHC class I mismatched barrier .
	manualset3
116900	8	404584	5	NULL	NULL	0	NULL	antigen presentation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings on host anti-donor alloresponse , as revealed by skin allograft survival and cytotoxic T lymphocyte assays , indicated that the administration of syngeneic DC presenting K ( bm1 ) donor-derived allopeptides through the indirect pathway of antigen presentation was not sufficient to induce cross-tolerance to alloreactive CD8 ( + ) T cells responding to bm1 alloantigens in a murine model of skin allograft transplantation across an MHC class I mismatched barrier .
	manualset3
116901	9	404584	5	NULL	NULL	0	NULL	cross-tolerance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings on host anti-donor alloresponse , as revealed by skin allograft survival and cytotoxic T lymphocyte assays , indicated that the administration of syngeneic DC presenting K ( bm1 ) donor-derived allopeptides through the indirect pathway of antigen presentation was not sufficient to induce cross-tolerance to alloreactive CD8 ( + ) T cells responding to bm1 alloantigens in a murine model of skin allograft transplantation across an MHC class I mismatched barrier .
	manualset3
116902	10	404584	5	NULL	NULL	0	NULL	alloreactive CD8 ( + ) T cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings on host anti-donor alloresponse , as revealed by skin allograft survival and cytotoxic T lymphocyte assays , indicated that the administration of syngeneic DC presenting K ( bm1 ) donor-derived allopeptides through the indirect pathway of antigen presentation was not sufficient to induce cross-tolerance to alloreactive CD8 ( + ) T cells responding to bm1 alloantigens in a murine model of skin allograft transplantation across an MHC class I mismatched barrier .
	manualset3
116903	11	404584	5	NULL	NULL	0	NULL	bm1 alloantigens	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings on host anti-donor alloresponse , as revealed by skin allograft survival and cytotoxic T lymphocyte assays , indicated that the administration of syngeneic DC presenting K ( bm1 ) donor-derived allopeptides through the indirect pathway of antigen presentation was not sufficient to induce cross-tolerance to alloreactive CD8 ( + ) T cells responding to bm1 alloantigens in a murine model of skin allograft transplantation across an MHC class I mismatched barrier .
	manualset3
116904	12	404584	5	NULL	NULL	0	NULL	murine model 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings on host anti-donor alloresponse , as revealed by skin allograft survival and cytotoxic T lymphocyte assays , indicated that the administration of syngeneic DC presenting K ( bm1 ) donor-derived allopeptides through the indirect pathway of antigen presentation was not sufficient to induce cross-tolerance to alloreactive CD8 ( + ) T cells responding to bm1 alloantigens in a murine model of skin allograft transplantation across an MHC class I mismatched barrier .
	manualset3
116905	13	404584	5	NULL	NULL	0	NULL	skin allograft transplantation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings on host anti-donor alloresponse , as revealed by skin allograft survival and cytotoxic T lymphocyte assays , indicated that the administration of syngeneic DC presenting K ( bm1 ) donor-derived allopeptides through the indirect pathway of antigen presentation was not sufficient to induce cross-tolerance to alloreactive CD8 ( + ) T cells responding to bm1 alloantigens in a murine model of skin allograft transplantation across an MHC class I mismatched barrier .
	manualset3
116906	14	404584	5	NULL	NULL	0	NULL	MHC class I mismatched barrier 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings on host anti-donor alloresponse , as revealed by skin allograft survival and cytotoxic T lymphocyte assays , indicated that the administration of syngeneic DC presenting K ( bm1 ) donor-derived allopeptides through the indirect pathway of antigen presentation was not sufficient to induce cross-tolerance to alloreactive CD8 ( + ) T cells responding to bm1 alloantigens in a murine model of skin allograft transplantation across an MHC class I mismatched barrier .
	manualset3
116907	1	404585	5	NULL	NULL	0	NULL	findings 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings strongly suggest that IGHMBP2 is a component of the translational machinery and that these components can be manipulated genetically to suppress motor neuron degeneration .
	manualset3
116908	2	404585	5	NULL	NULL	0	NULL	IGHMBP2 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings strongly suggest that IGHMBP2 is a component of the translational machinery and that these components can be manipulated genetically to suppress motor neuron degeneration .
	manualset3
116909	3	404585	5	NULL	NULL	0	NULL	component 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings strongly suggest that IGHMBP2 is a component of the translational machinery and that these components can be manipulated genetically to suppress motor neuron degeneration .
	manualset3
116910	4	404585	5	NULL	NULL	NULL	NULL	translational machinery	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our findings strongly suggest that IGHMBP2 is a component of the translational machinery and that these components can be manipulated genetically to suppress motor neuron degeneration .
	manualset3
116911	5	404585	5	NULL	NULL	0	NULL	components 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings strongly suggest that IGHMBP2 is a component of the translational machinery and that these components can be manipulated genetically to suppress motor neuron degeneration .
	manualset3
116912	6	404585	5	NULL	NULL	0	NULL	motor neuron degeneration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our findings strongly suggest that IGHMBP2 is a component of the translational machinery and that these components can be manipulated genetically to suppress motor neuron degeneration .
	manualset3
116913	1	404586	5	NULL	NULL	0	NULL	gene expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our gene expression results in MES3 cells were partially confirmed in CGR8 cells , showing numerous genes that are expressed in both mouse stem cells .
	manualset3
116914	2	404586	5	NULL	NULL	0	NULL	MES3 cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our gene expression results in MES3 cells were partially confirmed in CGR8 cells , showing numerous genes that are expressed in both mouse stem cells .
	manualset3
116915	3	404586	5	NULL	NULL	0	NULL	CGR8 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our gene expression results in MES3 cells were partially confirmed in CGR8 cells , showing numerous genes that are expressed in both mouse stem cells .
	manualset3
116916	4	404586	5	NULL	NULL	0	NULL	numerous genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our gene expression results in MES3 cells were partially confirmed in CGR8 cells , showing numerous genes that are expressed in both mouse stem cells .
	manualset3
116917	5	404586	5	NULL	NULL	0	NULL	mouse stem cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our gene expression results in MES3 cells were partially confirmed in CGR8 cells , showing numerous genes that are expressed in both mouse stem cells .
	manualset3
116918	1	404587	5	NULL	NULL	0	NULL	idea 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our idea is to systematically increase the size of the training set according to the desired basin of attraction around each prototype vector .
	manualset3
116919	2	404587	5	NULL	NULL	0	NULL	size 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our idea is to systematically increase the size of the training set according to the desired basin of attraction around each prototype vector .
	manualset3
116920	3	404587	5	NULL	NULL	0	NULL	training set	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our idea is to systematically increase the size of the training set according to the desired basin of attraction around each prototype vector .
	manualset3
116921	4	404587	5	NULL	NULL	0	NULL	desired basin 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our idea is to systematically increase the size of the training set according to the desired basin of attraction around each prototype vector .
	manualset3
116922	5	404587	5	NULL	NULL	0	NULL	attraction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our idea is to systematically increase the size of the training set according to the desired basin of attraction around each prototype vector .
	manualset3
116923	6	404587	5	NULL	NULL	NULL	NULL	prototype vector	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our idea is to systematically increase the size of the training set according to the desired basin of attraction around each prototype vector .
	manualset3
116924	1	404588	5	NULL	NULL	0	NULL	identification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our identification of Kek5 as a modulator of BMP signaling supports the emerging notion that LIG proteins function as diverse regulators of cellular communication .
	manualset3
116925	2	404588	5	NULL	NULL	0	NULL	Kek5 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our identification of Kek5 as a modulator of BMP signaling supports the emerging notion that LIG proteins function as diverse regulators of cellular communication .
	manualset3
116926	3	404588	5	NULL	NULL	0	NULL	modulator 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our identification of Kek5 as a modulator of BMP signaling supports the emerging notion that LIG proteins function as diverse regulators of cellular communication .
	manualset3
116927	4	404588	5	NULL	NULL	0	NULL	BMP signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our identification of Kek5 as a modulator of BMP signaling supports the emerging notion that LIG proteins function as diverse regulators of cellular communication .
	manualset3
116928	5	404588	5	NULL	NULL	0	NULL	emerging notion 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our identification of Kek5 as a modulator of BMP signaling supports the emerging notion that LIG proteins function as diverse regulators of cellular communication .
	manualset3
116929	6	404588	5	NULL	NULL	0	NULL	LIG proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our identification of Kek5 as a modulator of BMP signaling supports the emerging notion that LIG proteins function as diverse regulators of cellular communication .
	manualset3
116930	7	404588	5	NULL	NULL	0	NULL	diverse regulators	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our identification of Kek5 as a modulator of BMP signaling supports the emerging notion that LIG proteins function as diverse regulators of cellular communication .
	manualset3
116931	8	404588	5	NULL	NULL	0	NULL	cellular communication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our identification of Kek5 as a modulator of BMP signaling supports the emerging notion that LIG proteins function as diverse regulators of cellular communication .
	manualset3
116932	1	404589	5	NULL	NULL	0	NULL	insight 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our insight into the association between NPHS2 variants and nephrotic disease is hampered by the limitations of the existing studies , including small numbers of affected individuals and suboptimal control groups .
	manualset3
116933	2	404589	5	NULL	NULL	NULL	NULL	association 	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our insight into the association between NPHS2 variants and nephrotic disease is hampered by the limitations of the existing studies , including small numbers of affected individuals and suboptimal control groups .
	manualset3
116934	3	404589	5	NULL	NULL	0	NULL	NPHS2 variants 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our insight into the association between NPHS2 variants and nephrotic disease is hampered by the limitations of the existing studies , including small numbers of affected individuals and suboptimal control groups .
	manualset3
116935	4	404589	5	NULL	NULL	0	NULL	nephrotic disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our insight into the association between NPHS2 variants and nephrotic disease is hampered by the limitations of the existing studies , including small numbers of affected individuals and suboptimal control groups .
	manualset3
116936	5	404589	5	NULL	NULL	0	NULL	limitations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our insight into the association between NPHS2 variants and nephrotic disease is hampered by the limitations of the existing studies , including small numbers of affected individuals and suboptimal control groups .
	manualset3
116937	6	404589	5	NULL	NULL	0	NULL	existing studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our insight into the association between NPHS2 variants and nephrotic disease is hampered by the limitations of the existing studies , including small numbers of affected individuals and suboptimal control groups .
	manualset3
116938	7	404589	5	NULL	NULL	0	NULL	ssmall numbers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our insight into the association between NPHS2 variants and nephrotic disease is hampered by the limitations of the existing studies , including small numbers of affected individuals and suboptimal control groups .
	manualset3
116939	8	404589	5	NULL	NULL	0	NULL	affected individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our insight into the association between NPHS2 variants and nephrotic disease is hampered by the limitations of the existing studies , including small numbers of affected individuals and suboptimal control groups .
	manualset3
116940	9	404589	5	NULL	NULL	0	NULL	suboptimal control groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our insight into the association between NPHS2 variants and nephrotic disease is hampered by the limitations of the existing studies , including small numbers of affected individuals and suboptimal control groups .
	manualset3
116941	1	404590	5	NULL	NULL	0	NULL	fatal case	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A fatal case of hypereosinophilic syndrome in a 16-year-old girl with petechiae , edema , urticaria , and diffuse erythema unfolded over 2 weeks .
	manualset3
116942	2	404590	5	NULL	NULL	0	NULL	hypereosinophilic syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A fatal case of hypereosinophilic syndrome in a 16-year-old girl with petechiae , edema , urticaria , and diffuse erythema unfolded over 2 weeks .
	manualset3
116943	3	404590	5	NULL	NULL	0	NULL	16-year-old girl	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A fatal case of hypereosinophilic syndrome in a 16-year-old girl with petechiae , edema , urticaria , and diffuse erythema unfolded over 2 weeks .
	manualset3
116944	4	404590	5	NULL	NULL	0	NULL	petechiae 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A fatal case of hypereosinophilic syndrome in a 16-year-old girl with petechiae , edema , urticaria , and diffuse erythema unfolded over 2 weeks .
	manualset3
116945	5	404590	5	NULL	NULL	0	NULL	edema 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A fatal case of hypereosinophilic syndrome in a 16-year-old girl with petechiae , edema , urticaria , and diffuse erythema unfolded over 2 weeks .
	manualset3
116946	6	404590	5	NULL	NULL	0	NULL	urticaria 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A fatal case of hypereosinophilic syndrome in a 16-year-old girl with petechiae , edema , urticaria , and diffuse erythema unfolded over 2 weeks .
	manualset3
116947	7	404590	5	NULL	NULL	0	NULL	diffuse erythema	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A fatal case of hypereosinophilic syndrome in a 16-year-old girl with petechiae , edema , urticaria , and diffuse erythema unfolded over 2 weeks .
	manualset3
116948	8	404590	5	NULL	NULL	0	NULL	2 weeks	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	A fatal case of hypereosinophilic syndrome in a 16-year-old girl with petechiae , edema , urticaria , and diffuse erythema unfolded over 2 weeks .
	manualset3
116949	1	404591	5	NULL	NULL	0	NULL	pilot study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our pilot study suggests an association of some variants of the cytokine genes ( e.g. , IL1A-889 ) with a predisposition to development of severe osteolysis .
	manualset3
116950	2	404591	5	NULL	NULL	0	NULL	association 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our pilot study suggests an association of some variants of the cytokine genes ( e.g. , IL1A-889 ) with a predisposition to development of severe osteolysis .
	manualset3
116951	3	404591	5	NULL	NULL	0	NULL	variants 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our pilot study suggests an association of some variants of the cytokine genes ( e.g. , IL1A-889 ) with a predisposition to development of severe osteolysis .
	manualset3
116952	4	404591	5	NULL	NULL	0	NULL	cytokine genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our pilot study suggests an association of some variants of the cytokine genes ( e.g. , IL1A-889 ) with a predisposition to development of severe osteolysis .
	manualset3
116953	5	404591	5	NULL	NULL	0	NULL	IL1A-889	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Our pilot study suggests an association of some variants of the cytokine genes ( e.g. , IL1A-889 ) with a predisposition to development of severe osteolysis .
	manualset3
116954	6	404591	5	NULL	NULL	0	NULL	predisposition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our pilot study suggests an association of some variants of the cytokine genes ( e.g. , IL1A-889 ) with a predisposition to development of severe osteolysis .
	manualset3
116955	7	404591	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our pilot study suggests an association of some variants of the cytokine genes ( e.g. , IL1A-889 ) with a predisposition to development of severe osteolysis .
	manualset3
116956	8	404591	5	NULL	NULL	0	NULL	severe osteolysis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our pilot study suggests an association of some variants of the cytokine genes ( e.g. , IL1A-889 ) with a predisposition to development of severe osteolysis .
	manualset3
116957	1	404592	5	NULL	NULL	0	NULL	immunologic assay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our preferred immunologic assay for cysticercosis is the enzyme-linked immunoelectrodifusion transfer blot , or immunoblot , using the lentil lectin bound antigens from larval cysts .
	manualset3
116958	2	404592	5	NULL	NULL	0	NULL	cysticercosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our preferred immunologic assay for cysticercosis is the enzyme-linked immunoelectrodifusion transfer blot , or immunoblot , using the lentil lectin bound antigens from larval cysts .
	manualset3
116959	3	404592	5	NULL	NULL	NULL	NULL	enzyme-linked immunoelectrodifusion transfer blot 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Our preferred immunologic assay for cysticercosis is the enzyme-linked immunoelectrodifusion transfer blot , or immunoblot , using the lentil lectin bound antigens from larval cysts .
	manualset3
116960	4	404592	5	NULL	NULL	0	NULL	immunoblot 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our preferred immunologic assay for cysticercosis is the enzyme-linked immunoelectrodifusion transfer blot , or immunoblot , using the lentil lectin bound antigens from larval cysts .
	manualset3
116961	5	404592	5	NULL	NULL	0	NULL	lentil lectin bound antigens	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Our preferred immunologic assay for cysticercosis is the enzyme-linked immunoelectrodifusion transfer blot , or immunoblot , using the lentil lectin bound antigens from larval cysts .
	manualset3
116962	6	404592	5	NULL	NULL	0	NULL	larval cysts	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our preferred immunologic assay for cysticercosis is the enzyme-linked immunoelectrodifusion transfer blot , or immunoblot , using the lentil lectin bound antigens from larval cysts .
	manualset3
116963	1	404593	5	NULL	NULL	0	NULL	preliminary data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our preliminary data indicate that superoxide radicals were detected in the brain after cold-induced injury , but free and PEG-SOD had no beneficial effect on vasogenic brain edema produced by cold-induced injury .
	manualset3
116964	2	404593	5	NULL	NULL	0	NULL	superoxide radicals 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Our preliminary data indicate that superoxide radicals were detected in the brain after cold-induced injury , but free and PEG-SOD had no beneficial effect on vasogenic brain edema produced by cold-induced injury .
	manualset3
116965	3	404593	5	NULL	NULL	0	NULL	brain 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our preliminary data indicate that superoxide radicals were detected in the brain after cold-induced injury , but free and PEG-SOD had no beneficial effect on vasogenic brain edema produced by cold-induced injury .
	manualset3
116966	4	404593	5	NULL	NULL	0	NULL	cold-induced injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our preliminary data indicate that superoxide radicals were detected in the brain after cold-induced injury , but free and PEG-SOD had no beneficial effect on vasogenic brain edema produced by cold-induced injury .
	manualset3
116967	5	404593	5	NULL	NULL	0	NULL	PEG-SOD	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our preliminary data indicate that superoxide radicals were detected in the brain after cold-induced injury , but free and PEG-SOD had no beneficial effect on vasogenic brain edema produced by cold-induced injury .
	manualset3
116968	6	404593	5	NULL	NULL	0	NULL	beneficial effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our preliminary data indicate that superoxide radicals were detected in the brain after cold-induced injury , but free and PEG-SOD had no beneficial effect on vasogenic brain edema produced by cold-induced injury .
	manualset3
116969	7	404593	5	NULL	NULL	0	NULL	vasogenic brain edema	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our preliminary data indicate that superoxide radicals were detected in the brain after cold-induced injury , but free and PEG-SOD had no beneficial effect on vasogenic brain edema produced by cold-induced injury .
	manualset3
116970	8	404593	5	NULL	NULL	0	NULL	cold-induced injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our preliminary data indicate that superoxide radicals were detected in the brain after cold-induced injury , but free and PEG-SOD had no beneficial effect on vasogenic brain edema produced by cold-induced injury .
	manualset3
116971	1	404594	5	NULL	NULL	0	NULL	present observation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our present observation that plasma ACTH was unchanged after ethanol intake , but plasma BE was increased at 0100-0200 hr may be due to the fact that our BE antiserum cross-reacts with beta-lipotropin , which has a considerably longer half-life than ACTH or BE , and also to the long sampling interval .
	manualset3
116972	2	404594	5	NULL	NULL	0	NULL	plasma ACTH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our present observation that plasma ACTH was unchanged after ethanol intake , but plasma BE was increased at 0100-0200 hr may be due to the fact that our BE antiserum cross-reacts with beta-lipotropin , which has a considerably longer half-life than ACTH or BE , and also to the long sampling interval .
	manualset3
116973	3	404594	5	NULL	NULL	0	NULL	ethanol intake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our present observation that plasma ACTH was unchanged after ethanol intake , but plasma BE was increased at 0100-0200 hr may be due to the fact that our BE antiserum cross-reacts with beta-lipotropin , which has a considerably longer half-life than ACTH or BE , and also to the long sampling interval .
	manualset3
116974	4	404594	5	NULL	NULL	0	NULL	plasma BE	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our present observation that plasma ACTH was unchanged after ethanol intake , but plasma BE was increased at 0100-0200 hr may be due to the fact that our BE antiserum cross-reacts with beta-lipotropin , which has a considerably longer half-life than ACTH or BE , and also to the long sampling interval .
	manualset3
116975	5	404594	5	NULL	NULL	0	NULL	0100-0200 hr 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our present observation that plasma ACTH was unchanged after ethanol intake , but plasma BE was increased at 0100-0200 hr may be due to the fact that our BE antiserum cross-reacts with beta-lipotropin , which has a considerably longer half-life than ACTH or BE , and also to the long sampling interval .
	manualset3
116976	6	404594	5	NULL	NULL	0	NULL	fact 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our present observation that plasma ACTH was unchanged after ethanol intake , but plasma BE was increased at 0100-0200 hr may be due to the fact that our BE antiserum cross-reacts with beta-lipotropin , which has a considerably longer half-life than ACTH or BE , and also to the long sampling interval .
	manualset3
116977	7	404594	5	NULL	NULL	0	NULL	BE antiserum 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Our present observation that plasma ACTH was unchanged after ethanol intake , but plasma BE was increased at 0100-0200 hr may be due to the fact that our BE antiserum cross-reacts with beta-lipotropin , which has a considerably longer half-life than ACTH or BE , and also to the long sampling interval .
	manualset3
116978	8	404594	5	NULL	NULL	0	NULL	beta-lipotropin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our present observation that plasma ACTH was unchanged after ethanol intake , but plasma BE was increased at 0100-0200 hr may be due to the fact that our BE antiserum cross-reacts with beta-lipotropin , which has a considerably longer half-life than ACTH or BE , and also to the long sampling interval .
	manualset3
116979	9	404594	5	NULL	NULL	0	NULL	longer half-life	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our present observation that plasma ACTH was unchanged after ethanol intake , but plasma BE was increased at 0100-0200 hr may be due to the fact that our BE antiserum cross-reacts with beta-lipotropin , which has a considerably longer half-life than ACTH or BE , and also to the long sampling interval .
	manualset3
116980	10	404594	5	NULL	NULL	0	NULL	ACTH 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our present observation that plasma ACTH was unchanged after ethanol intake , but plasma BE was increased at 0100-0200 hr may be due to the fact that our BE antiserum cross-reacts with beta-lipotropin , which has a considerably longer half-life than ACTH or BE , and also to the long sampling interval .
	manualset3
116981	11	404594	5	NULL	NULL	0	NULL	BE 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our present observation that plasma ACTH was unchanged after ethanol intake , but plasma BE was increased at 0100-0200 hr may be due to the fact that our BE antiserum cross-reacts with beta-lipotropin , which has a considerably longer half-life than ACTH or BE , and also to the long sampling interval .
	manualset3
116982	12	404594	5	NULL	NULL	0	NULL	long sampling interval	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Our present observation that plasma ACTH was unchanged after ethanol intake , but plasma BE was increased at 0100-0200 hr may be due to the fact that our BE antiserum cross-reacts with beta-lipotropin , which has a considerably longer half-life than ACTH or BE , and also to the long sampling interval .
	manualset3
116983	1	404595	5	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our present study indicates that further developments and future benefits of fetoscopy entirely depend on the progress of laboratory techniques which can provide more accurate data through specimens obtained fetoscopy .
	manualset3
116984	2	404595	5	NULL	NULL	0	NULL	further developments 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our present study indicates that further developments and future benefits of fetoscopy entirely depend on the progress of laboratory techniques which can provide more accurate data through specimens obtained fetoscopy .
	manualset3
116985	3	404595	5	NULL	NULL	0	NULL	future benefits	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our present study indicates that further developments and future benefits of fetoscopy entirely depend on the progress of laboratory techniques which can provide more accurate data through specimens obtained fetoscopy .
	manualset3
116986	4	404595	5	NULL	NULL	0	NULL	fetoscopy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our present study indicates that further developments and future benefits of fetoscopy entirely depend on the progress of laboratory techniques which can provide more accurate data through specimens obtained fetoscopy .
	manualset3
116987	5	404595	5	NULL	NULL	0	NULL	progress 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our present study indicates that further developments and future benefits of fetoscopy entirely depend on the progress of laboratory techniques which can provide more accurate data through specimens obtained fetoscopy .
	manualset3
116988	6	404595	5	NULL	NULL	0	NULL	laboratory techniques 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our present study indicates that further developments and future benefits of fetoscopy entirely depend on the progress of laboratory techniques which can provide more accurate data through specimens obtained fetoscopy .
	manualset3
116989	7	404595	5	NULL	NULL	0	NULL	accurate data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our present study indicates that further developments and future benefits of fetoscopy entirely depend on the progress of laboratory techniques which can provide more accurate data through specimens obtained fetoscopy .
	manualset3
116990	8	404595	5	NULL	NULL	0	NULL	specimens 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our present study indicates that further developments and future benefits of fetoscopy entirely depend on the progress of laboratory techniques which can provide more accurate data through specimens obtained fetoscopy .
	manualset3
116991	9	404595	5	NULL	NULL	0	NULL	fetoscopy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our present study indicates that further developments and future benefits of fetoscopy entirely depend on the progress of laboratory techniques which can provide more accurate data through specimens obtained fetoscopy .
	manualset3
116992	1	404596	5	NULL	NULL	0	NULL	previous results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our previous and present results strongly suggest that indole compounds , which are involved in the regulation of various neuroendocrine processes in fish , are synthetized within the CRL .
	manualset3
116993	2	404596	5	NULL	NULL	0	NULL	present results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our previous and present results strongly suggest that indole compounds , which are involved in the regulation of various neuroendocrine processes in fish , are synthetized within the CRL .
	manualset3
116994	3	404596	5	NULL	NULL	0	NULL	indole compounds	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Our previous and present results strongly suggest that indole compounds , which are involved in the regulation of various neuroendocrine processes in fish , are synthetized within the CRL .
	manualset3
116995	4	404596	5	NULL	NULL	0	NULL	regulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our previous and present results strongly suggest that indole compounds , which are involved in the regulation of various neuroendocrine processes in fish , are synthetized within the CRL .
	manualset3
116996	5	404596	5	NULL	NULL	0	NULL	neuroendocrine processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our previous and present results strongly suggest that indole compounds , which are involved in the regulation of various neuroendocrine processes in fish , are synthetized within the CRL .
	manualset3
116997	6	404596	5	NULL	NULL	0	NULL	fish 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our previous and present results strongly suggest that indole compounds , which are involved in the regulation of various neuroendocrine processes in fish , are synthetized within the CRL .
	manualset3
116998	7	404596	5	NULL	NULL	0	NULL	CRL 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our previous and present results strongly suggest that indole compounds , which are involved in the regulation of various neuroendocrine processes in fish , are synthetized within the CRL .
	manualset3
116999	1	404597	5	NULL	NULL	0	NULL	previous studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our previous studies have demonstrated that addition of moderate volumes of absolute alcohol ( 34-170 mM final concentration ) to whole blood produces concentration-dependent platelet aggregation , due to release of adenosine diphosphate ( ADP ) from erythrocytes .
	manualset3
117000	2	404597	5	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our previous studies have demonstrated that addition of moderate volumes of absolute alcohol ( 34-170 mM final concentration ) to whole blood produces concentration-dependent platelet aggregation , due to release of adenosine diphosphate ( ADP ) from erythrocytes .
	manualset3
117001	3	404597	5	NULL	NULL	0	NULL	moderate volumes 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our previous studies have demonstrated that addition of moderate volumes of absolute alcohol ( 34-170 mM final concentration ) to whole blood produces concentration-dependent platelet aggregation , due to release of adenosine diphosphate ( ADP ) from erythrocytes .
	manualset3
117002	4	404597	5	NULL	NULL	0	NULL	absolute alcohol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our previous studies have demonstrated that addition of moderate volumes of absolute alcohol ( 34-170 mM final concentration ) to whole blood produces concentration-dependent platelet aggregation , due to release of adenosine diphosphate ( ADP ) from erythrocytes .
	manualset3
117003	5	404597	5	NULL	NULL	0	NULL	34-170 mM final concentration 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our previous studies have demonstrated that addition of moderate volumes of absolute alcohol ( 34-170 mM final concentration ) to whole blood produces concentration-dependent platelet aggregation , due to release of adenosine diphosphate ( ADP ) from erythrocytes .
	manualset3
117004	6	404597	5	NULL	NULL	0	NULL	whole blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Our previous studies have demonstrated that addition of moderate volumes of absolute alcohol ( 34-170 mM final concentration ) to whole blood produces concentration-dependent platelet aggregation , due to release of adenosine diphosphate ( ADP ) from erythrocytes .
	manualset3
117005	7	404597	5	NULL	NULL	0	NULL	concentration-dependent platelet aggregation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our previous studies have demonstrated that addition of moderate volumes of absolute alcohol ( 34-170 mM final concentration ) to whole blood produces concentration-dependent platelet aggregation , due to release of adenosine diphosphate ( ADP ) from erythrocytes .
	manualset3
117006	8	404597	5	NULL	NULL	0	NULL	release 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our previous studies have demonstrated that addition of moderate volumes of absolute alcohol ( 34-170 mM final concentration ) to whole blood produces concentration-dependent platelet aggregation , due to release of adenosine diphosphate ( ADP ) from erythrocytes .
	manualset3
117007	9	404597	5	NULL	NULL	0	NULL	adenosine diphosphate ( ADP )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Our previous studies have demonstrated that addition of moderate volumes of absolute alcohol ( 34-170 mM final concentration ) to whole blood produces concentration-dependent platelet aggregation , due to release of adenosine diphosphate ( ADP ) from erythrocytes .
	manualset3
117008	10	404597	5	NULL	NULL	0	NULL	erythrocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our previous studies have demonstrated that addition of moderate volumes of absolute alcohol ( 34-170 mM final concentration ) to whole blood produces concentration-dependent platelet aggregation , due to release of adenosine diphosphate ( ADP ) from erythrocytes .
	manualset3
117009	1	404598	5	NULL	NULL	0	NULL	DAT-selective piperidine analog , 4 - ( 2 - ( diphenylmethoxy ) ethyl ) -1 - benzylpiperidine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Our previously developed DAT-selective piperidine analog , 4 - ( 2 - ( diphenylmethoxy ) ethyl ) -1 - benzylpiperidine , was the basis for our current structure-activity relationship ( SAR ) studies exploring the significance of the contribution of the benzhydryl O - and N-atoms in these molecules in interacting with the DAT .
	manualset3
117010	2	404598	5	NULL	NULL	0	NULL	current structure-activity relationship ( SAR ) studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our previously developed DAT-selective piperidine analog , 4 - ( 2 - ( diphenylmethoxy ) ethyl ) -1 - benzylpiperidine , was the basis for our current structure-activity relationship ( SAR ) studies exploring the significance of the contribution of the benzhydryl O - and N-atoms in these molecules in interacting with the DAT .
	manualset3
117011	3	404598	5	NULL	NULL	0	NULL	significance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our previously developed DAT-selective piperidine analog , 4 - ( 2 - ( diphenylmethoxy ) ethyl ) -1 - benzylpiperidine , was the basis for our current structure-activity relationship ( SAR ) studies exploring the significance of the contribution of the benzhydryl O - and N-atoms in these molecules in interacting with the DAT .
	manualset3
117012	4	404598	5	NULL	NULL	0	NULL	contribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our previously developed DAT-selective piperidine analog , 4 - ( 2 - ( diphenylmethoxy ) ethyl ) -1 - benzylpiperidine , was the basis for our current structure-activity relationship ( SAR ) studies exploring the significance of the contribution of the benzhydryl O - and N-atoms in these molecules in interacting with the DAT .
	manualset3
117013	5	404598	5	NULL	NULL	0	NULL	benzhydryl O -atoms	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Our previously developed DAT-selective piperidine analog , 4 - ( 2 - ( diphenylmethoxy ) ethyl ) -1 - benzylpiperidine , was the basis for our current structure-activity relationship ( SAR ) studies exploring the significance of the contribution of the benzhydryl O - and N-atoms in these molecules in interacting with the DAT .
	manualset3
117014	6	404598	5	NULL	NULL	0	NULL	benzhydryl N -atoms	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Our previously developed DAT-selective piperidine analog , 4 - ( 2 - ( diphenylmethoxy ) ethyl ) -1 - benzylpiperidine , was the basis for our current structure-activity relationship ( SAR ) studies exploring the significance of the contribution of the benzhydryl O - and N-atoms in these molecules in interacting with the DAT .
	manualset3
117015	7	404598	5	NULL	NULL	0	NULL	molecules 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Our previously developed DAT-selective piperidine analog , 4 - ( 2 - ( diphenylmethoxy ) ethyl ) -1 - benzylpiperidine , was the basis for our current structure-activity relationship ( SAR ) studies exploring the significance of the contribution of the benzhydryl O - and N-atoms in these molecules in interacting with the DAT .
	manualset3
117016	8	404598	5	NULL	NULL	0	NULL	DAT 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our previously developed DAT-selective piperidine analog , 4 - ( 2 - ( diphenylmethoxy ) ethyl ) -1 - benzylpiperidine , was the basis for our current structure-activity relationship ( SAR ) studies exploring the significance of the contribution of the benzhydryl O - and N-atoms in these molecules in interacting with the DAT .
	manualset3
117017	1	404599	5	NULL	NULL	0	NULL	father 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A father and his daughter with Birt-Hogg-Dub-syndrome were treated with the CO2 laser , producing satisfactory results .
	manualset3
117018	2	404599	5	NULL	NULL	0	NULL	daughter 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A father and his daughter with Birt-Hogg-Dub-syndrome were treated with the CO2 laser , producing satisfactory results .
	manualset3
117019	3	404599	5	NULL	NULL	0	NULL	Birt-Hogg-Dub-syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A father and his daughter with Birt-Hogg-Dub-syndrome were treated with the CO2 laser , producing satisfactory results .
	manualset3
117020	4	404599	5	NULL	NULL	0	NULL	CO2 laser 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	A father and his daughter with Birt-Hogg-Dub-syndrome were treated with the CO2 laser , producing satisfactory results .
	manualset3
117021	5	404599	5	NULL	NULL	0	NULL	satisfactory results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A father and his daughter with Birt-Hogg-Dub-syndrome were treated with the CO2 laser , producing satisfactory results .
	manualset3
117022	1	404600	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our recent data suggested that the improved effectiveness of insulin that occurs as a result of physical exercise is attributable , at least in part , to increases in GLUT4 protein , IRS1 and PI3-kinase protein in skeletal muscle .
	manualset3
117023	2	404600	5	NULL	NULL	0	NULL	improved effectiveness 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our recent data suggested that the improved effectiveness of insulin that occurs as a result of physical exercise is attributable , at least in part , to increases in GLUT4 protein , IRS1 and PI3-kinase protein in skeletal muscle .
	manualset3
117024	3	404600	5	NULL	NULL	0	NULL	insulin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our recent data suggested that the improved effectiveness of insulin that occurs as a result of physical exercise is attributable , at least in part , to increases in GLUT4 protein , IRS1 and PI3-kinase protein in skeletal muscle .
	manualset3
117025	4	404600	5	NULL	NULL	0	NULL	result 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our recent data suggested that the improved effectiveness of insulin that occurs as a result of physical exercise is attributable , at least in part , to increases in GLUT4 protein , IRS1 and PI3-kinase protein in skeletal muscle .
	manualset3
117026	5	404600	5	NULL	NULL	0	NULL	physical exercise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our recent data suggested that the improved effectiveness of insulin that occurs as a result of physical exercise is attributable , at least in part , to increases in GLUT4 protein , IRS1 and PI3-kinase protein in skeletal muscle .
	manualset3
117027	6	404600	5	NULL	NULL	0	NULL	GLUT4 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our recent data suggested that the improved effectiveness of insulin that occurs as a result of physical exercise is attributable , at least in part , to increases in GLUT4 protein , IRS1 and PI3-kinase protein in skeletal muscle .
	manualset3
117028	7	404600	5	NULL	NULL	0	NULL	IRS1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our recent data suggested that the improved effectiveness of insulin that occurs as a result of physical exercise is attributable , at least in part , to increases in GLUT4 protein , IRS1 and PI3-kinase protein in skeletal muscle .
	manualset3
117029	8	404600	5	NULL	NULL	0	NULL	PI3-kinase protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our recent data suggested that the improved effectiveness of insulin that occurs as a result of physical exercise is attributable , at least in part , to increases in GLUT4 protein , IRS1 and PI3-kinase protein in skeletal muscle .
	manualset3
117030	9	404600	5	NULL	NULL	0	NULL	skeletal muscle 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Our recent data suggested that the improved effectiveness of insulin that occurs as a result of physical exercise is attributable , at least in part , to increases in GLUT4 protein , IRS1 and PI3-kinase protein in skeletal muscle .
	manualset3
117031	1	404601	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results also indicate that the global protein features contribute little to the formation and prediction of disulfide bonds , while the local sequential and structural information play important roles .
	manualset3
117032	2	404601	5	NULL	NULL	0	NULL	global protein features	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results also indicate that the global protein features contribute little to the formation and prediction of disulfide bonds , while the local sequential and structural information play important roles .
	manualset3
117033	3	404601	5	NULL	NULL	0	NULL	formation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results also indicate that the global protein features contribute little to the formation and prediction of disulfide bonds , while the local sequential and structural information play important roles .
	manualset3
117034	4	404601	5	NULL	NULL	0	NULL	prediction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results also indicate that the global protein features contribute little to the formation and prediction of disulfide bonds , while the local sequential and structural information play important roles .
	manualset3
117035	5	404601	5	NULL	NULL	0	NULL	disulfide bonds	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results also indicate that the global protein features contribute little to the formation and prediction of disulfide bonds , while the local sequential and structural information play important roles .
	manualset3
117036	6	404601	5	NULL	NULL	0	NULL	local sequential information	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results also indicate that the global protein features contribute little to the formation and prediction of disulfide bonds , while the local sequential and structural information play important roles .
	manualset3
117037	7	404601	5	NULL	NULL	0	NULL	structural information	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results also indicate that the global protein features contribute little to the formation and prediction of disulfide bonds , while the local sequential and structural information play important roles .
	manualset3
117038	8	404601	5	NULL	NULL	0	NULL	important roles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results also indicate that the global protein features contribute little to the formation and prediction of disulfide bonds , while the local sequential and structural information play important roles .
	manualset3
117039	1	404602	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results also show that , in contrast to the other algorithms , PhyloGibbs can make realistic estimates of the reliability of its predictions .
	manualset3
117040	2	404602	5	NULL	NULL	0	NULL	algorithms 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results also show that , in contrast to the other algorithms , PhyloGibbs can make realistic estimates of the reliability of its predictions .
	manualset3
117041	3	404602	5	NULL	NULL	0	NULL	PhyloGibbs 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results also show that , in contrast to the other algorithms , PhyloGibbs can make realistic estimates of the reliability of its predictions .
	manualset3
117042	4	404602	5	NULL	NULL	0	NULL	reliability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results also show that , in contrast to the other algorithms , PhyloGibbs can make realistic estimates of the reliability of its predictions .
	manualset3
117043	5	404602	5	NULL	NULL	0	NULL	predictions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results also show that , in contrast to the other algorithms , PhyloGibbs can make realistic estimates of the reliability of its predictions .
	manualset3
117044	1	404603	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results also suggest that SP in the rostral NTS does not play a direct role in mediating the cardiovascular responses to unloading the carotid baroreceptors .
	manualset3
117045	2	404603	5	NULL	NULL	0	NULL	SP 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results also suggest that SP in the rostral NTS does not play a direct role in mediating the cardiovascular responses to unloading the carotid baroreceptors .
	manualset3
117046	3	404603	5	NULL	NULL	0	NULL	rostral NTS	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results also suggest that SP in the rostral NTS does not play a direct role in mediating the cardiovascular responses to unloading the carotid baroreceptors .
	manualset3
117047	4	404603	5	NULL	NULL	0	NULL	direct role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results also suggest that SP in the rostral NTS does not play a direct role in mediating the cardiovascular responses to unloading the carotid baroreceptors .
	manualset3
117048	5	404603	5	NULL	NULL	0	NULL	cardiovascular responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results also suggest that SP in the rostral NTS does not play a direct role in mediating the cardiovascular responses to unloading the carotid baroreceptors .
	manualset3
117049	6	404603	5	NULL	NULL	0	NULL	carotid baroreceptors	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results also suggest that SP in the rostral NTS does not play a direct role in mediating the cardiovascular responses to unloading the carotid baroreceptors .
	manualset3
117050	1	404604	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results strongly suggest that p21 and p27 , related Cdk inhibitors , select their cell cycle regulatory Cdk targets by binding specifically to the cyclin subunit of these Cdk/cyclin complexes as a first step in a sequential , folding-on-binding mechanism .
	manualset3
117051	2	404604	5	NULL	NULL	0	NULL	p21	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results strongly suggest that p21 and p27 , related Cdk inhibitors , select their cell cycle regulatory Cdk targets by binding specifically to the cyclin subunit of these Cdk/cyclin complexes as a first step in a sequential , folding-on-binding mechanism .
	manualset3
117052	3	404604	5	NULL	NULL	0	NULL	p27	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results strongly suggest that p21 and p27 , related Cdk inhibitors , select their cell cycle regulatory Cdk targets by binding specifically to the cyclin subunit of these Cdk/cyclin complexes as a first step in a sequential , folding-on-binding mechanism .
	manualset3
117053	4	404604	5	NULL	NULL	0	NULL	Cdk inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results strongly suggest that p21 and p27 , related Cdk inhibitors , select their cell cycle regulatory Cdk targets by binding specifically to the cyclin subunit of these Cdk/cyclin complexes as a first step in a sequential , folding-on-binding mechanism .
	manualset3
117054	5	404604	5	NULL	NULL	0	NULL	cell cycle regulatory Cdk targets	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results strongly suggest that p21 and p27 , related Cdk inhibitors , select their cell cycle regulatory Cdk targets by binding specifically to the cyclin subunit of these Cdk/cyclin complexes as a first step in a sequential , folding-on-binding mechanism .
	manualset3
117055	6	404604	5	NULL	NULL	0	NULL	cyclin subunit	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results strongly suggest that p21 and p27 , related Cdk inhibitors , select their cell cycle regulatory Cdk targets by binding specifically to the cyclin subunit of these Cdk/cyclin complexes as a first step in a sequential , folding-on-binding mechanism .
	manualset3
117056	7	404604	5	NULL	NULL	0	NULL	Cdk/cyclin complexes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results strongly suggest that p21 and p27 , related Cdk inhibitors , select their cell cycle regulatory Cdk targets by binding specifically to the cyclin subunit of these Cdk/cyclin complexes as a first step in a sequential , folding-on-binding mechanism .
	manualset3
117057	8	404604	5	NULL	NULL	0	NULL	first step	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results strongly suggest that p21 and p27 , related Cdk inhibitors , select their cell cycle regulatory Cdk targets by binding specifically to the cyclin subunit of these Cdk/cyclin complexes as a first step in a sequential , folding-on-binding mechanism .
	manualset3
117058	9	404604	5	NULL	NULL	0	NULL	sequential , folding-on-binding mechanism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results strongly suggest that p21 and p27 , related Cdk inhibitors , select their cell cycle regulatory Cdk targets by binding specifically to the cyclin subunit of these Cdk/cyclin complexes as a first step in a sequential , folding-on-binding mechanism .
	manualset3
117059	1	404605	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results together with those reported in literature indicated that this epitope resides in the highly divergent region of amino acid residues 525 to 540 .
	manualset3
117060	2	404605	5	NULL	NULL	0	NULL	literature 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results together with those reported in literature indicated that this epitope resides in the highly divergent region of amino acid residues 525 to 540 .
	manualset3
117061	3	404605	5	NULL	NULL	0	NULL	epitope 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results together with those reported in literature indicated that this epitope resides in the highly divergent region of amino acid residues 525 to 540 .
	manualset3
117062	4	404605	5	NULL	NULL	0	NULL	highly divergent region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results together with those reported in literature indicated that this epitope resides in the highly divergent region of amino acid residues 525 to 540 .
	manualset3
117063	5	404605	5	NULL	NULL	0	NULL	amino acid residues 525 to 540	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results together with those reported in literature indicated that this epitope resides in the highly divergent region of amino acid residues 525 to 540 .
	manualset3
117064	1	404606	5	NULL	NULL	0	NULL	revised test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our revised test ( 1997 ) takes into account the quantitative factor of success , as well as the qualitative factor of movement planning .
	manualset3
117065	2	404606	5	NULL	NULL	0	NULL	1997 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Our revised test ( 1997 ) takes into account the quantitative factor of success , as well as the qualitative factor of movement planning .
	manualset3
117066	3	404606	5	NULL	NULL	0	NULL	quantitative factor	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our revised test ( 1997 ) takes into account the quantitative factor of success , as well as the qualitative factor of movement planning .
	manualset3
117067	4	404606	5	NULL	NULL	0	NULL	success 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our revised test ( 1997 ) takes into account the quantitative factor of success , as well as the qualitative factor of movement planning .
	manualset3
117068	5	404606	5	NULL	NULL	0	NULL	qualitative factor 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our revised test ( 1997 ) takes into account the quantitative factor of success , as well as the qualitative factor of movement planning .
	manualset3
117069	6	404606	5	NULL	NULL	0	NULL	movement planning 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our revised test ( 1997 ) takes into account the quantitative factor of success , as well as the qualitative factor of movement planning .
	manualset3
117070	1	404607	5	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies involving five normal bulls of proven fertility , two SCNT-derived bulls , and four mature offspring of SCNT bulls showed that the mean number of crossing over per spermatocyte for normal bulls ( 42 + / - 4 SD ; ranging from 33 to 56 ) , was not significantly different from that of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 35 to 56 ) , and the offspring of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 37 to 58 ) .
	manualset3
117071	2	404607	5	NULL	NULL	0	NULL	five 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies involving five normal bulls of proven fertility , two SCNT-derived bulls , and four mature offspring of SCNT bulls showed that the mean number of crossing over per spermatocyte for normal bulls ( 42 + / - 4 SD ; ranging from 33 to 56 ) , was not significantly different from that of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 35 to 56 ) , and the offspring of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 37 to 58 ) .
	manualset3
117072	3	404607	5	NULL	NULL	0	NULL	normal bulls 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies involving five normal bulls of proven fertility , two SCNT-derived bulls , and four mature offspring of SCNT bulls showed that the mean number of crossing over per spermatocyte for normal bulls ( 42 + / - 4 SD ; ranging from 33 to 56 ) , was not significantly different from that of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 35 to 56 ) , and the offspring of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 37 to 58 ) .
	manualset3
117073	4	404607	5	NULL	NULL	0	NULL	proven fertility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies involving five normal bulls of proven fertility , two SCNT-derived bulls , and four mature offspring of SCNT bulls showed that the mean number of crossing over per spermatocyte for normal bulls ( 42 + / - 4 SD ; ranging from 33 to 56 ) , was not significantly different from that of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 35 to 56 ) , and the offspring of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 37 to 58 ) .
	manualset3
117074	5	404607	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies involving five normal bulls of proven fertility , two SCNT-derived bulls , and four mature offspring of SCNT bulls showed that the mean number of crossing over per spermatocyte for normal bulls ( 42 + / - 4 SD ; ranging from 33 to 56 ) , was not significantly different from that of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 35 to 56 ) , and the offspring of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 37 to 58 ) .
	manualset3
117075	6	404607	5	NULL	NULL	0	NULL	SCNT-derived bulls	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies involving five normal bulls of proven fertility , two SCNT-derived bulls , and four mature offspring of SCNT bulls showed that the mean number of crossing over per spermatocyte for normal bulls ( 42 + / - 4 SD ; ranging from 33 to 56 ) , was not significantly different from that of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 35 to 56 ) , and the offspring of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 37 to 58 ) .
	manualset3
117076	7	404607	5	NULL	NULL	0	NULL	four 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies involving five normal bulls of proven fertility , two SCNT-derived bulls , and four mature offspring of SCNT bulls showed that the mean number of crossing over per spermatocyte for normal bulls ( 42 + / - 4 SD ; ranging from 33 to 56 ) , was not significantly different from that of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 35 to 56 ) , and the offspring of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 37 to 58 ) .
	manualset3
117077	8	404607	5	NULL	NULL	0	NULL	mature offspring	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies involving five normal bulls of proven fertility , two SCNT-derived bulls , and four mature offspring of SCNT bulls showed that the mean number of crossing over per spermatocyte for normal bulls ( 42 + / - 4 SD ; ranging from 33 to 56 ) , was not significantly different from that of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 35 to 56 ) , and the offspring of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 37 to 58 ) .
	manualset3
117078	9	404607	5	NULL	NULL	0	NULL	SCNT bulls	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies involving five normal bulls of proven fertility , two SCNT-derived bulls , and four mature offspring of SCNT bulls showed that the mean number of crossing over per spermatocyte for normal bulls ( 42 + / - 4 SD ; ranging from 33 to 56 ) , was not significantly different from that of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 35 to 56 ) , and the offspring of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 37 to 58 ) .
	manualset3
117079	10	404607	5	NULL	NULL	0	NULL	mean number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies involving five normal bulls of proven fertility , two SCNT-derived bulls , and four mature offspring of SCNT bulls showed that the mean number of crossing over per spermatocyte for normal bulls ( 42 + / - 4 SD ; ranging from 33 to 56 ) , was not significantly different from that of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 35 to 56 ) , and the offspring of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 37 to 58 ) .
	manualset3
117080	11	404607	5	NULL	NULL	0	NULL	crossing over	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies involving five normal bulls of proven fertility , two SCNT-derived bulls , and four mature offspring of SCNT bulls showed that the mean number of crossing over per spermatocyte for normal bulls ( 42 + / - 4 SD ; ranging from 33 to 56 ) , was not significantly different from that of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 35 to 56 ) , and the offspring of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 37 to 58 ) .
	manualset3
117081	12	404607	5	NULL	NULL	0	NULL	spermatocyte 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies involving five normal bulls of proven fertility , two SCNT-derived bulls , and four mature offspring of SCNT bulls showed that the mean number of crossing over per spermatocyte for normal bulls ( 42 + / - 4 SD ; ranging from 33 to 56 ) , was not significantly different from that of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 35 to 56 ) , and the offspring of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 37 to 58 ) .
	manualset3
117082	13	404607	5	NULL	NULL	0	NULL	normal bulls 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies involving five normal bulls of proven fertility , two SCNT-derived bulls , and four mature offspring of SCNT bulls showed that the mean number of crossing over per spermatocyte for normal bulls ( 42 + / - 4 SD ; ranging from 33 to 56 ) , was not significantly different from that of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 35 to 56 ) , and the offspring of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 37 to 58 ) .
	manualset3
117083	14	404607	5	NULL	NULL	0	NULL	42 + / - 4 SD	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies involving five normal bulls of proven fertility , two SCNT-derived bulls , and four mature offspring of SCNT bulls showed that the mean number of crossing over per spermatocyte for normal bulls ( 42 + / - 4 SD ; ranging from 33 to 56 ) , was not significantly different from that of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 35 to 56 ) , and the offspring of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 37 to 58 ) .
	manualset3
117084	15	404607	5	NULL	NULL	0	NULL	33 to 56	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies involving five normal bulls of proven fertility , two SCNT-derived bulls , and four mature offspring of SCNT bulls showed that the mean number of crossing over per spermatocyte for normal bulls ( 42 + / - 4 SD ; ranging from 33 to 56 ) , was not significantly different from that of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 35 to 56 ) , and the offspring of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 37 to 58 ) .
	manualset3
117085	16	404607	5	NULL	NULL	0	NULL	SCNT-derived bulls	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies involving five normal bulls of proven fertility , two SCNT-derived bulls , and four mature offspring of SCNT bulls showed that the mean number of crossing over per spermatocyte for normal bulls ( 42 + / - 4 SD ; ranging from 33 to 56 ) , was not significantly different from that of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 35 to 56 ) , and the offspring of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 37 to 58 ) .
	manualset3
117086	17	404607	5	NULL	NULL	0	NULL	43 + / - 5 SD	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies involving five normal bulls of proven fertility , two SCNT-derived bulls , and four mature offspring of SCNT bulls showed that the mean number of crossing over per spermatocyte for normal bulls ( 42 + / - 4 SD ; ranging from 33 to 56 ) , was not significantly different from that of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 35 to 56 ) , and the offspring of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 37 to 58 ) .
	manualset3
117087	18	404607	5	NULL	NULL	0	NULL	35 to 56	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies involving five normal bulls of proven fertility , two SCNT-derived bulls , and four mature offspring of SCNT bulls showed that the mean number of crossing over per spermatocyte for normal bulls ( 42 + / - 4 SD ; ranging from 33 to 56 ) , was not significantly different from that of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 35 to 56 ) , and the offspring of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 37 to 58 ) .
	manualset3
117088	19	404607	5	NULL	NULL	0	NULL	offspring 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies involving five normal bulls of proven fertility , two SCNT-derived bulls , and four mature offspring of SCNT bulls showed that the mean number of crossing over per spermatocyte for normal bulls ( 42 + / - 4 SD ; ranging from 33 to 56 ) , was not significantly different from that of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 35 to 56 ) , and the offspring of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 37 to 58 ) .
	manualset3
117089	20	404607	5	NULL	NULL	0	NULL	SCNT-derived bulls 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies involving five normal bulls of proven fertility , two SCNT-derived bulls , and four mature offspring of SCNT bulls showed that the mean number of crossing over per spermatocyte for normal bulls ( 42 + / - 4 SD ; ranging from 33 to 56 ) , was not significantly different from that of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 35 to 56 ) , and the offspring of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 37 to 58 ) .
	manualset3
117090	21	404607	5	NULL	NULL	0	NULL	43 + / - 5 SD	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies involving five normal bulls of proven fertility , two SCNT-derived bulls , and four mature offspring of SCNT bulls showed that the mean number of crossing over per spermatocyte for normal bulls ( 42 + / - 4 SD ; ranging from 33 to 56 ) , was not significantly different from that of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 35 to 56 ) , and the offspring of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 37 to 58 ) .
	manualset3
117091	22	404607	5	NULL	NULL	0	NULL	37 to 58	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Our studies involving five normal bulls of proven fertility , two SCNT-derived bulls , and four mature offspring of SCNT bulls showed that the mean number of crossing over per spermatocyte for normal bulls ( 42 + / - 4 SD ; ranging from 33 to 56 ) , was not significantly different from that of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 35 to 56 ) , and the offspring of SCNT-derived bulls ( 43 + / - 5 SD ; ranging from 37 to 58 ) .
	manualset3
117092	1	404608	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study demonstrates that the use of different primer pairs generate significant differences in DGGE analysis of enterococcal population , consequently , appropriate primers regarding the purpose of analysis can be selected .
	manualset3
117093	2	404608	5	NULL	NULL	0	NULL	use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study demonstrates that the use of different primer pairs generate significant differences in DGGE analysis of enterococcal population , consequently , appropriate primers regarding the purpose of analysis can be selected .
	manualset3
117094	3	404608	5	NULL	NULL	0	NULL	primer pairs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study demonstrates that the use of different primer pairs generate significant differences in DGGE analysis of enterococcal population , consequently , appropriate primers regarding the purpose of analysis can be selected .
	manualset3
117095	4	404608	5	NULL	NULL	0	NULL	DGGE analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study demonstrates that the use of different primer pairs generate significant differences in DGGE analysis of enterococcal population , consequently , appropriate primers regarding the purpose of analysis can be selected .
	manualset3
117096	5	404608	5	NULL	NULL	0	NULL	enterococcal population 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study demonstrates that the use of different primer pairs generate significant differences in DGGE analysis of enterococcal population , consequently , appropriate primers regarding the purpose of analysis can be selected .
	manualset3
117097	6	404608	5	NULL	NULL	0	NULL	appropriate primers	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study demonstrates that the use of different primer pairs generate significant differences in DGGE analysis of enterococcal population , consequently , appropriate primers regarding the purpose of analysis can be selected .
	manualset3
117098	7	404608	5	NULL	NULL	0	NULL	purpose 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study demonstrates that the use of different primer pairs generate significant differences in DGGE analysis of enterococcal population , consequently , appropriate primers regarding the purpose of analysis can be selected .
	manualset3
117099	8	404608	5	NULL	NULL	0	NULL	analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study demonstrates that the use of different primer pairs generate significant differences in DGGE analysis of enterococcal population , consequently , appropriate primers regarding the purpose of analysis can be selected .
	manualset3
117100	1	404609	5	NULL	NULL	0	NULL	favourable effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A favourable effect on bronchial hyper-reactivity and on delayed hypersensitivity reactions has also been observed .
	manualset3
117101	2	404609	5	NULL	NULL	0	NULL	bronchial hyper-reactivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A favourable effect on bronchial hyper-reactivity and on delayed hypersensitivity reactions has also been observed .
	manualset3
117102	3	404609	5	NULL	NULL	0	NULL	delayed hypersensitivity reactions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A favourable effect on bronchial hyper-reactivity and on delayed hypersensitivity reactions has also been observed .
	manualset3
117103	1	404610	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study further showed that the SPC gene expression level in differentiated cells was related to the ratio of BMSCs to MRC-5 cells and the components of modified SAGM .
	manualset3
117104	2	404610	5	NULL	NULL	0	NULL	SPC gene expression level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study further showed that the SPC gene expression level in differentiated cells was related to the ratio of BMSCs to MRC-5 cells and the components of modified SAGM .
	manualset3
117105	3	404610	5	NULL	NULL	0	NULL	differentiated cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study further showed that the SPC gene expression level in differentiated cells was related to the ratio of BMSCs to MRC-5 cells and the components of modified SAGM .
	manualset3
117106	4	404610	5	NULL	NULL	0	NULL	ratio 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study further showed that the SPC gene expression level in differentiated cells was related to the ratio of BMSCs to MRC-5 cells and the components of modified SAGM .
	manualset3
117107	5	404610	5	NULL	NULL	0	NULL	BMSCs 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study further showed that the SPC gene expression level in differentiated cells was related to the ratio of BMSCs to MRC-5 cells and the components of modified SAGM .
	manualset3
117108	6	404610	5	NULL	NULL	0	NULL	MRC-5 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study further showed that the SPC gene expression level in differentiated cells was related to the ratio of BMSCs to MRC-5 cells and the components of modified SAGM .
	manualset3
117109	7	404610	5	NULL	NULL	0	NULL	components 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study further showed that the SPC gene expression level in differentiated cells was related to the ratio of BMSCs to MRC-5 cells and the components of modified SAGM .
	manualset3
117110	8	404610	5	NULL	NULL	0	NULL	modified SAGM	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study further showed that the SPC gene expression level in differentiated cells was related to the ratio of BMSCs to MRC-5 cells and the components of modified SAGM .
	manualset3
117111	1	404611	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study indicates also that NS5 is an adequate target region to differentiate HCV strains derived from different patients in the same hospital .
	manualset3
117112	2	404611	5	NULL	NULL	0	NULL	NS5 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study indicates also that NS5 is an adequate target region to differentiate HCV strains derived from different patients in the same hospital .
	manualset3
117113	3	404611	5	NULL	NULL	0	NULL	adequate target region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study indicates also that NS5 is an adequate target region to differentiate HCV strains derived from different patients in the same hospital .
	manualset3
117114	4	404611	5	NULL	NULL	0	NULL	HCV strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study indicates also that NS5 is an adequate target region to differentiate HCV strains derived from different patients in the same hospital .
	manualset3
117115	5	404611	5	NULL	NULL	0	NULL	different patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study indicates also that NS5 is an adequate target region to differentiate HCV strains derived from different patients in the same hospital .
	manualset3
117116	6	404611	5	NULL	NULL	0	NULL	hospital 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study indicates also that NS5 is an adequate target region to differentiate HCV strains derived from different patients in the same hospital .
	manualset3
117117	1	404612	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study of these cases supports the existence of the CHARGE-association ( Coloboma , Heart Disease , Atresia of choanae , Retarded mental development and growth , Genital hypoplasia , Ear anomalies and deafness ) .
	manualset3
117118	2	404612	5	NULL	NULL	0	NULL	cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study of these cases supports the existence of the CHARGE-association ( Coloboma , Heart Disease , Atresia of choanae , Retarded mental development and growth , Genital hypoplasia , Ear anomalies and deafness ) .
	manualset3
117119	3	404612	5	NULL	NULL	0	NULL	existence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study of these cases supports the existence of the CHARGE-association ( Coloboma , Heart Disease , Atresia of choanae , Retarded mental development and growth , Genital hypoplasia , Ear anomalies and deafness ) .
	manualset3
117120	4	404612	5	NULL	NULL	0	NULL	CHARGE-association ( Coloboma , Heart Disease , Atresia of choanae , Retarded mental development and growth , Genital hypoplasia , Ear anomalies and deafness )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study of these cases supports the existence of the CHARGE-association ( Coloboma , Heart Disease , Atresia of choanae , Retarded mental development and growth , Genital hypoplasia , Ear anomalies and deafness ) .
	manualset3
117121	1	404613	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study reveals that coprolites can be an interesting source of parasites that can be readily identified using molecular approaches .
	manualset3
117122	2	404613	5	NULL	NULL	0	NULL	coprolites 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study reveals that coprolites can be an interesting source of parasites that can be readily identified using molecular approaches .
	manualset3
117123	3	404613	5	NULL	NULL	0	NULL	source 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study reveals that coprolites can be an interesting source of parasites that can be readily identified using molecular approaches .
	manualset3
117124	4	404613	5	NULL	NULL	0	NULL	parasites 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study reveals that coprolites can be an interesting source of parasites that can be readily identified using molecular approaches .
	manualset3
117125	5	404613	5	NULL	NULL	0	NULL	molecular approaches	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study reveals that coprolites can be an interesting source of parasites that can be readily identified using molecular approaches .
	manualset3
117126	1	404614	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study shows a variety of neuropathological findings as the etiology .
	manualset3
117127	2	404614	5	NULL	NULL	0	NULL	variety 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study shows a variety of neuropathological findings as the etiology .
	manualset3
117128	3	404614	5	NULL	NULL	0	NULL	neuropathological findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study shows a variety of neuropathological findings as the etiology .
	manualset3
117129	4	404614	5	NULL	NULL	0	NULL	etiology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study shows a variety of neuropathological findings as the etiology .
	manualset3
117130	1	404615	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study suggests that - elemene is a promising drug to enhance tumor radioresponse , and survivin and HIF-1 are novel targets of - elemene .
	manualset3
117131	2	404615	5	NULL	NULL	0	NULL	elemene 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study suggests that - elemene is a promising drug to enhance tumor radioresponse , and survivin and HIF-1 are novel targets of - elemene .
	manualset3
117132	3	404615	5	NULL	NULL	0	NULL	promising drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study suggests that - elemene is a promising drug to enhance tumor radioresponse , and survivin and HIF-1 are novel targets of - elemene .
	manualset3
117133	4	404615	5	NULL	NULL	0	NULL	tumor radioresponse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study suggests that - elemene is a promising drug to enhance tumor radioresponse , and survivin and HIF-1 are novel targets of - elemene .
	manualset3
117134	5	404615	5	NULL	NULL	0	NULL	survivin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study suggests that - elemene is a promising drug to enhance tumor radioresponse , and survivin and HIF-1 are novel targets of - elemene .
	manualset3
117135	6	404615	5	NULL	NULL	0	NULL	HIF-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study suggests that - elemene is a promising drug to enhance tumor radioresponse , and survivin and HIF-1 are novel targets of - elemene .
	manualset3
117136	7	404615	5	NULL	NULL	0	NULL	novel targets 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study suggests that - elemene is a promising drug to enhance tumor radioresponse , and survivin and HIF-1 are novel targets of - elemene .
	manualset3
117137	8	404615	5	NULL	NULL	0	NULL	elemene 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study suggests that - elemene is a promising drug to enhance tumor radioresponse , and survivin and HIF-1 are novel targets of - elemene .
	manualset3
117138	1	404616	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study suggests that workers in the fur manufacturing industry develop acute and chronic respiratory problems often associated with specific indicators of atopy .
	manualset3
117139	2	404616	5	NULL	NULL	0	NULL	workers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study suggests that workers in the fur manufacturing industry develop acute and chronic respiratory problems often associated with specific indicators of atopy .
	manualset3
117140	3	404616	5	NULL	NULL	0	NULL	fur manufacturing industry 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study suggests that workers in the fur manufacturing industry develop acute and chronic respiratory problems often associated with specific indicators of atopy .
	manualset3
117141	4	404616	5	NULL	NULL	0	NULL	acute respiratory problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study suggests that workers in the fur manufacturing industry develop acute and chronic respiratory problems often associated with specific indicators of atopy .
	manualset3
117142	5	404616	5	NULL	NULL	0	NULL	chronic respiratory problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study suggests that workers in the fur manufacturing industry develop acute and chronic respiratory problems often associated with specific indicators of atopy .
	manualset3
117143	6	404616	5	NULL	NULL	0	NULL	specific indicators	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study suggests that workers in the fur manufacturing industry develop acute and chronic respiratory problems often associated with specific indicators of atopy .
	manualset3
117144	7	404616	5	NULL	NULL	0	NULL	atopy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our study suggests that workers in the fur manufacturing industry develop acute and chronic respiratory problems often associated with specific indicators of atopy .
	manualset3
117145	1	404617	5	NULL	NULL	0	NULL	success rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our success rate using the HA-coated prosthesis is similar to previous reports that used antibiotic impregnated bone cement .
	manualset3
117146	2	404617	5	NULL	NULL	0	NULL	HA-coated prosthesis	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Our success rate using the HA-coated prosthesis is similar to previous reports that used antibiotic impregnated bone cement .
	manualset3
117147	3	404617	5	NULL	NULL	0	NULL	reports 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our success rate using the HA-coated prosthesis is similar to previous reports that used antibiotic impregnated bone cement .
	manualset3
117148	4	404617	5	NULL	NULL	0	NULL	antibiotic impregnated bone cement	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our success rate using the HA-coated prosthesis is similar to previous reports that used antibiotic impregnated bone cement .
	manualset3
117149	1	404618	5	NULL	NULL	0	NULL	time-frequency analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our time-frequency analysis on physiological tremor data revealed that tremor contains multiple dominant frequencies over the entire duration rather than a single dominant frequency .
	manualset3
117150	2	404618	5	NULL	NULL	0	NULL	physiological tremor data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our time-frequency analysis on physiological tremor data revealed that tremor contains multiple dominant frequencies over the entire duration rather than a single dominant frequency .
	manualset3
117151	3	404618	5	NULL	NULL	0	NULL	tremor 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our time-frequency analysis on physiological tremor data revealed that tremor contains multiple dominant frequencies over the entire duration rather than a single dominant frequency .
	manualset3
117152	4	404618	5	NULL	NULL	0	NULL	multiple dominant frequencies	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our time-frequency analysis on physiological tremor data revealed that tremor contains multiple dominant frequencies over the entire duration rather than a single dominant frequency .
	manualset3
117153	5	404618	5	NULL	NULL	0	NULL	duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Our time-frequency analysis on physiological tremor data revealed that tremor contains multiple dominant frequencies over the entire duration rather than a single dominant frequency .
	manualset3
117154	6	404618	5	NULL	NULL	0	NULL	single dominant frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our time-frequency analysis on physiological tremor data revealed that tremor contains multiple dominant frequencies over the entire duration rather than a single dominant frequency .
	manualset3
117155	1	404619	5	NULL	NULL	0	NULL	work 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work has considerable clinical relevance , since it may enable the earlier diagnosis of aggressive PCa through routine biopsy assessment of eNOS , ERbeta , and HIF-2alpha expression .
	manualset3
117156	2	404619	5	NULL	NULL	0	NULL	clinical relevance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work has considerable clinical relevance , since it may enable the earlier diagnosis of aggressive PCa through routine biopsy assessment of eNOS , ERbeta , and HIF-2alpha expression .
	manualset3
117157	3	404619	5	NULL	NULL	0	NULL	earlier diagnosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work has considerable clinical relevance , since it may enable the earlier diagnosis of aggressive PCa through routine biopsy assessment of eNOS , ERbeta , and HIF-2alpha expression .
	manualset3
117158	4	404619	5	NULL	NULL	0	NULL	aggressive PCa	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work has considerable clinical relevance , since it may enable the earlier diagnosis of aggressive PCa through routine biopsy assessment of eNOS , ERbeta , and HIF-2alpha expression .
	manualset3
117159	5	404619	5	NULL	NULL	0	NULL	routine biopsy assessment 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work has considerable clinical relevance , since it may enable the earlier diagnosis of aggressive PCa through routine biopsy assessment of eNOS , ERbeta , and HIF-2alpha expression .
	manualset3
117160	6	404619	5	NULL	NULL	0	NULL	eNOS expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work has considerable clinical relevance , since it may enable the earlier diagnosis of aggressive PCa through routine biopsy assessment of eNOS , ERbeta , and HIF-2alpha expression .
	manualset3
117161	7	404619	5	NULL	NULL	0	NULL	ERbeta expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work has considerable clinical relevance , since it may enable the earlier diagnosis of aggressive PCa through routine biopsy assessment of eNOS , ERbeta , and HIF-2alpha expression .
	manualset3
117162	8	404619	5	NULL	NULL	0	NULL	HIF-2alpha expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work has considerable clinical relevance , since it may enable the earlier diagnosis of aggressive PCa through routine biopsy assessment of eNOS , ERbeta , and HIF-2alpha expression .
	manualset3
117163	1	404620	5	NULL	NULL	0	NULL	work 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work has led to the identification of the defective genes in three forms of limb girdle muscular dystrophy ( LGMD ) and a better understanding of how muscle degenerates in many of the different dystrophies .
	manualset3
117164	2	404620	5	NULL	NULL	0	NULL	identification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work has led to the identification of the defective genes in three forms of limb girdle muscular dystrophy ( LGMD ) and a better understanding of how muscle degenerates in many of the different dystrophies .
	manualset3
117165	3	404620	5	NULL	NULL	0	NULL	defective genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work has led to the identification of the defective genes in three forms of limb girdle muscular dystrophy ( LGMD ) and a better understanding of how muscle degenerates in many of the different dystrophies .
	manualset3
117166	4	404620	5	NULL	NULL	0	NULL	three forms	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work has led to the identification of the defective genes in three forms of limb girdle muscular dystrophy ( LGMD ) and a better understanding of how muscle degenerates in many of the different dystrophies .
	manualset3
117167	5	404620	5	NULL	NULL	0	NULL	limb girdle muscular dystrophy ( LGMD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work has led to the identification of the defective genes in three forms of limb girdle muscular dystrophy ( LGMD ) and a better understanding of how muscle degenerates in many of the different dystrophies .
	manualset3
117168	6	404620	5	NULL	NULL	0	NULL	understanding 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work has led to the identification of the defective genes in three forms of limb girdle muscular dystrophy ( LGMD ) and a better understanding of how muscle degenerates in many of the different dystrophies .
	manualset3
117169	7	404620	5	NULL	NULL	0	NULL	muscle 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work has led to the identification of the defective genes in three forms of limb girdle muscular dystrophy ( LGMD ) and a better understanding of how muscle degenerates in many of the different dystrophies .
	manualset3
117170	8	404620	5	NULL	NULL	0	NULL	different dystrophies 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work has led to the identification of the defective genes in three forms of limb girdle muscular dystrophy ( LGMD ) and a better understanding of how muscle degenerates in many of the different dystrophies .
	manualset3
117171	1	404621	5	NULL	NULL	0	NULL	work 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work highlights the challenges encountered on using the simple model along with postmortem data to infer iron content in several brain regions where postmortem iron data are scant ( e.g. , corpus callosum , amygdale ) .
	manualset3
117172	2	404621	5	NULL	NULL	0	NULL	challenges 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work highlights the challenges encountered on using the simple model along with postmortem data to infer iron content in several brain regions where postmortem iron data are scant ( e.g. , corpus callosum , amygdale ) .
	manualset3
117173	3	404621	5	NULL	NULL	0	NULL	simple model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work highlights the challenges encountered on using the simple model along with postmortem data to infer iron content in several brain regions where postmortem iron data are scant ( e.g. , corpus callosum , amygdale ) .
	manualset3
117174	4	404621	5	NULL	NULL	0	NULL	postmortem data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work highlights the challenges encountered on using the simple model along with postmortem data to infer iron content in several brain regions where postmortem iron data are scant ( e.g. , corpus callosum , amygdale ) .
	manualset3
117175	5	404621	5	NULL	NULL	0	NULL	iron content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work highlights the challenges encountered on using the simple model along with postmortem data to infer iron content in several brain regions where postmortem iron data are scant ( e.g. , corpus callosum , amygdale ) .
	manualset3
117176	6	404621	5	NULL	NULL	0	NULL	several brain regions	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work highlights the challenges encountered on using the simple model along with postmortem data to infer iron content in several brain regions where postmortem iron data are scant ( e.g. , corpus callosum , amygdale ) .
	manualset3
117177	7	404621	5	NULL	NULL	0	NULL	postmortem iron data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work highlights the challenges encountered on using the simple model along with postmortem data to infer iron content in several brain regions where postmortem iron data are scant ( e.g. , corpus callosum , amygdale ) .
	manualset3
117178	8	404621	5	NULL	NULL	0	NULL	corpus callosum	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work highlights the challenges encountered on using the simple model along with postmortem data to infer iron content in several brain regions where postmortem iron data are scant ( e.g. , corpus callosum , amygdale ) .
	manualset3
117179	9	404621	5	NULL	NULL	0	NULL	amygdale 	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work highlights the challenges encountered on using the simple model along with postmortem data to infer iron content in several brain regions where postmortem iron data are scant ( e.g. , corpus callosum , amygdale ) .
	manualset3
117180	1	404622	5	NULL	NULL	0	NULL	work 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work lays the groundwork for developing stimulus-responsive VNPs that can be used as `` smart '' building blocks for the creation of higher order structures .
	manualset3
117181	2	404622	5	NULL	NULL	0	NULL	groundwork 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work lays the groundwork for developing stimulus-responsive VNPs that can be used as `` smart '' building blocks for the creation of higher order structures .
	manualset3
117182	3	404622	5	NULL	NULL	0	NULL	stimulus-responsive VNPs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work lays the groundwork for developing stimulus-responsive VNPs that can be used as `` smart '' building blocks for the creation of higher order structures .
	manualset3
117183	4	404622	5	NULL	NULL	0	NULL	building blocks 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work lays the groundwork for developing stimulus-responsive VNPs that can be used as `` smart '' building blocks for the creation of higher order structures .
	manualset3
117184	5	404622	5	NULL	NULL	0	NULL	creation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work lays the groundwork for developing stimulus-responsive VNPs that can be used as `` smart '' building blocks for the creation of higher order structures .
	manualset3
117185	6	404622	5	NULL	NULL	0	NULL	higher order structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our work lays the groundwork for developing stimulus-responsive VNPs that can be used as `` smart '' building blocks for the creation of higher order structures .
	manualset3
117186	1	404623	5	NULL	NULL	0	NULL	20 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Out of 20 biopsy proven fibroadenoma tissues , 19 ( 95 % ) showed positivity for hNIS protein and only one was negative .
	manualset3
117187	2	404623	5	NULL	NULL	0	NULL	biopsy proven fibroadenoma tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Out of 20 biopsy proven fibroadenoma tissues , 19 ( 95 % ) showed positivity for hNIS protein and only one was negative .
	manualset3
117188	3	404623	5	NULL	NULL	0	NULL	19 ( 95 % ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Out of 20 biopsy proven fibroadenoma tissues , 19 ( 95 % ) showed positivity for hNIS protein and only one was negative .
	manualset3
117189	4	404623	5	NULL	NULL	0	NULL	hNIS protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Out of 20 biopsy proven fibroadenoma tissues , 19 ( 95 % ) showed positivity for hNIS protein and only one was negative .
	manualset3
117190	1	404624	5	NULL	NULL	0	NULL	8 , 878	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Out of the 8 , 878 births , 660 ( 7.5 % ) were of low birth weight .
	manualset3
117191	2	404624	5	NULL	NULL	0	NULL	births 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Out of the 8 , 878 births , 660 ( 7.5 % ) were of low birth weight .
	manualset3
117192	3	404624	5	NULL	NULL	0	NULL	660 ( 7.5 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Out of the 8 , 878 births , 660 ( 7.5 % ) were of low birth weight .
	manualset3
117193	4	404624	5	NULL	NULL	0	NULL	low birth weight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Out of the 8 , 878 births , 660 ( 7.5 % ) were of low birth weight .
	manualset3
117194	1	404625	5	NULL	NULL	0	NULL	feather abnormality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A feather abnormality in chicks fed diets deficient in certain amino acids .
	manualset3
117195	2	404625	5	NULL	NULL	0	NULL	chicks 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A feather abnormality in chicks fed diets deficient in certain amino acids .
	manualset3
117196	3	404625	5	NULL	NULL	0	NULL	diets 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A feather abnormality in chicks fed diets deficient in certain amino acids .
	manualset3
117197	4	404625	5	NULL	NULL	0	NULL	amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A feather abnormality in chicks fed diets deficient in certain amino acids .
	manualset3
117198	1	404626	5	NULL	NULL	0	NULL	Outcome measures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcome measures related to cardiac arrest are difficult to evaluate or compare because there have been no uniform definitions or uniform agreements on what data to report .
	manualset3
117199	2	404626	5	NULL	NULL	0	NULL	cardiac arrest	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcome measures related to cardiac arrest are difficult to evaluate or compare because there have been no uniform definitions or uniform agreements on what data to report .
	manualset3
117200	3	404626	5	NULL	NULL	0	NULL	evaluate 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcome measures related to cardiac arrest are difficult to evaluate or compare because there have been no uniform definitions or uniform agreements on what data to report .
	manualset3
117201	4	404626	5	NULL	NULL	0	NULL	compare 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcome measures related to cardiac arrest are difficult to evaluate or compare because there have been no uniform definitions or uniform agreements on what data to report .
	manualset3
117202	5	404626	5	NULL	NULL	0	NULL	uniform definitions 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcome measures related to cardiac arrest are difficult to evaluate or compare because there have been no uniform definitions or uniform agreements on what data to report .
	manualset3
117203	6	404626	5	NULL	NULL	0	NULL	uniform agreements	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcome measures related to cardiac arrest are difficult to evaluate or compare because there have been no uniform definitions or uniform agreements on what data to report .
	manualset3
117204	7	404626	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcome measures related to cardiac arrest are difficult to evaluate or compare because there have been no uniform definitions or uniform agreements on what data to report .
	manualset3
117205	8	404626	5	NULL	NULL	NULL	NULL	report 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Outcome measures related to cardiac arrest are difficult to evaluate or compare because there have been no uniform definitions or uniform agreements on what data to report .
	manualset3
117206	1	404627	5	NULL	NULL	NULL	NULL	Outcome 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Outcome of pregnancy from day 0 to 19 and serum tocopherol levels in mother rats fed on a rapeseed protein concentrate essentially free from glucosinolates .
	manualset3
117207	2	404627	5	NULL	NULL	0	NULL	pregnancy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcome of pregnancy from day 0 to 19 and serum tocopherol levels in mother rats fed on a rapeseed protein concentrate essentially free from glucosinolates .
	manualset3
117208	3	404627	5	NULL	NULL	0	NULL	day 0 to 19 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcome of pregnancy from day 0 to 19 and serum tocopherol levels in mother rats fed on a rapeseed protein concentrate essentially free from glucosinolates .
	manualset3
117209	4	404627	5	NULL	NULL	0	NULL	serum tocopherol levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcome of pregnancy from day 0 to 19 and serum tocopherol levels in mother rats fed on a rapeseed protein concentrate essentially free from glucosinolates .
	manualset3
117210	5	404627	5	NULL	NULL	0	NULL	mother rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcome of pregnancy from day 0 to 19 and serum tocopherol levels in mother rats fed on a rapeseed protein concentrate essentially free from glucosinolates .
	manualset3
117211	6	404627	5	NULL	NULL	0	NULL	rapeseed protein concentrate 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcome of pregnancy from day 0 to 19 and serum tocopherol levels in mother rats fed on a rapeseed protein concentrate essentially free from glucosinolates .
	manualset3
117212	7	404627	5	NULL	NULL	0	NULL	glucosinolates 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcome of pregnancy from day 0 to 19 and serum tocopherol levels in mother rats fed on a rapeseed protein concentrate essentially free from glucosinolates .
	manualset3
117213	1	404628	5	NULL	NULL	0	NULL	Outcomes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcomes after LTM in patients who had both epileptic seizures and nonepileptic seizures demonstrated that the epileptic seizures usually were controlled with medications .
	manualset3
117214	2	404628	5	NULL	NULL	0	NULL	LTM 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcomes after LTM in patients who had both epileptic seizures and nonepileptic seizures demonstrated that the epileptic seizures usually were controlled with medications .
	manualset3
117215	3	404628	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcomes after LTM in patients who had both epileptic seizures and nonepileptic seizures demonstrated that the epileptic seizures usually were controlled with medications .
	manualset3
117216	4	404628	5	NULL	NULL	0	NULL	epileptic seizures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcomes after LTM in patients who had both epileptic seizures and nonepileptic seizures demonstrated that the epileptic seizures usually were controlled with medications .
	manualset3
117230	7	404628	5	NULL	NULL	NULL	NULL	medications 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Outcomes after LTM in patients who had both epileptic seizures and nonepileptic seizures demonstrated that the epileptic seizures usually were controlled with medications .
	manualset3
121231	5	404628	5	NULL	NULL	0	NULL	nonepileptic seizures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcomes after LTM in patients who had both epileptic seizures and nonepileptic seizures demonstrated that the epileptic seizures usually were controlled with medications .
	manualset3
121232	6	404628	5	NULL	NULL	0	NULL	epileptic seizures 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcomes after LTM in patients who had both epileptic seizures and nonepileptic seizures demonstrated that the epileptic seizures usually were controlled with medications .
	manualset3
117231	1	404629	5	NULL	NULL	NULL	NULL	Outcomes 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Outcomes of advanced trauma life support training : questioning the role of observer .
	manualset3
117232	2	404629	5	NULL	NULL	0	NULL	advanced trauma life support training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcomes of advanced trauma life support training : questioning the role of observer .
	manualset3
117233	3	404629	5	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcomes of advanced trauma life support training : questioning the role of observer .
	manualset3
117234	4	404629	5	NULL	NULL	0	NULL	observer 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcomes of advanced trauma life support training : questioning the role of observer .
	manualset3
117235	1	404630	5	NULL	NULL	0	NULL	Outcomes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcomes of management of early temporomandibular joint disorders : How effective is nonsurgical therapy in the long-term ?
	manualset3
117236	2	404630	5	NULL	NULL	0	NULL	management 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcomes of management of early temporomandibular joint disorders : How effective is nonsurgical therapy in the long-term ?
	manualset3
117237	3	404630	5	NULL	NULL	0	NULL	early temporomandibular joint disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcomes of management of early temporomandibular joint disorders : How effective is nonsurgical therapy in the long-term ?
	manualset3
117240	4	404630	5	NULL	NULL	0	NULL	nonsurgical therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcomes of management of early temporomandibular joint disorders : How effective is nonsurgical therapy in the long-term ?
	manualset3
117242	5	404630	5	NULL	NULL	0	NULL	long-term	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcomes of management of early temporomandibular joint disorders : How effective is nonsurgical therapy in the long-term ?
	manualset3
117401	1	404631	5	NULL	NULL	0	NULL	Outer parenchyma	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Outer parenchyma and sapwood density ranged from 320 to 410 kg m ( -3 ) and from 420 to 620 kg m ( -3 ) , respectively , depending on the species .
	manualset3
117402	2	404631	5	NULL	NULL	0	NULL	sapwood density 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Outer parenchyma and sapwood density ranged from 320 to 410 kg m ( -3 ) and from 420 to 620 kg m ( -3 ) , respectively , depending on the species .
	manualset3
117403	3	404631	5	NULL	NULL	0	NULL	320 to 410 kg m ( -3 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Outer parenchyma and sapwood density ranged from 320 to 410 kg m ( -3 ) and from 420 to 620 kg m ( -3 ) , respectively , depending on the species .
	manualset3
117404	4	404631	5	NULL	NULL	0	NULL	420 to 620 kg m ( -3 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Outer parenchyma and sapwood density ranged from 320 to 410 kg m ( -3 ) and from 420 to 620 kg m ( -3 ) , respectively , depending on the species .
	manualset3
117405	5	404631	5	NULL	NULL	0	NULL	species 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Outer parenchyma and sapwood density ranged from 320 to 410 kg m ( -3 ) and from 420 to 620 kg m ( -3 ) , respectively , depending on the species .
	manualset3
117417	1	404632	5	NULL	NULL	0	NULL	Outlines 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Outlines of the modern diagnostics and therapy of the intracranial hypertension are presented .
	manualset3
117418	2	404632	5	NULL	NULL	0	NULL	modern diagnostics	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Outlines of the modern diagnostics and therapy of the intracranial hypertension are presented .
	manualset3
117419	3	404632	5	NULL	NULL	0	NULL	therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Outlines of the modern diagnostics and therapy of the intracranial hypertension are presented .
	manualset3
117420	4	404632	5	NULL	NULL	0	NULL	intracranial hypertension 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Outlines of the modern diagnostics and therapy of the intracranial hypertension are presented .
	manualset3
117421	1	404633	5	NULL	NULL	0	NULL	feeding episode	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A feeding episode is proposed to occur during an episode of increased sympathetic nervous system activity that stimulates BAT thermogenesis and increases body temperature .
	manualset3
117422	2	404633	5	NULL	NULL	NULL	NULL	episode 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A feeding episode is proposed to occur during an episode of increased sympathetic nervous system activity that stimulates BAT thermogenesis and increases body temperature .
	manualset3
117423	3	404633	5	NULL	NULL	0	NULL	increased sympathetic nervous system activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A feeding episode is proposed to occur during an episode of increased sympathetic nervous system activity that stimulates BAT thermogenesis and increases body temperature .
	manualset3
117424	4	404633	5	NULL	NULL	0	NULL	BAT thermogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A feeding episode is proposed to occur during an episode of increased sympathetic nervous system activity that stimulates BAT thermogenesis and increases body temperature .
	manualset3
117425	5	404633	5	NULL	NULL	0	NULL	body temperature	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A feeding episode is proposed to occur during an episode of increased sympathetic nervous system activity that stimulates BAT thermogenesis and increases body temperature .
	manualset3
117426	1	404634	5	NULL	NULL	0	NULL	Outpatient or `` ambulatory '' anesthesia	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Outpatient or `` ambulatory '' anesthesia and surgery has revolutionized the way surgery is practiced in the United States .
	manualset3
117427	2	404634	5	NULL	NULL	0	NULL	surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Outpatient or `` ambulatory '' anesthesia and surgery has revolutionized the way surgery is practiced in the United States .
	manualset3
117428	3	404634	5	NULL	NULL	0	NULL	surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Outpatient or `` ambulatory '' anesthesia and surgery has revolutionized the way surgery is practiced in the United States .
	manualset3
117429	4	404634	5	NULL	NULL	0	NULL	United States	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Outpatient or `` ambulatory '' anesthesia and surgery has revolutionized the way surgery is practiced in the United States .
	manualset3
117477	1	404635	5	NULL	NULL	0	NULL	Output inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Output inhibition upon application or programming head .
	manualset3
117478	2	404635	5	NULL	NULL	0	NULL	application 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Output inhibition upon application or programming head .
	manualset3
117490	3	404635	5	NULL	NULL	0	NULL	programming head	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Output inhibition upon application or programming head .
	manualset3
117494	1	404636	5	NULL	NULL	0	NULL	Ovalbumin glycopeptide fraction AC-C	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Ovalbumin glycopeptide fraction AC-C has been separated into at least four distinct glycopeptides .
	manualset3
117495	2	404636	5	NULL	NULL	0	NULL	four 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ovalbumin glycopeptide fraction AC-C has been separated into at least four distinct glycopeptides .
	manualset3
117496	3	404636	5	NULL	NULL	0	NULL	glycopeptides 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Ovalbumin glycopeptide fraction AC-C has been separated into at least four distinct glycopeptides .
	manualset3
117497	1	404637	5	NULL	NULL	0	NULL	Ovariectomized mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ovariectomized mice were treated with estrogen and progesterone on a schedule to mimic early pregnancy .
	manualset3
117498	2	404637	5	NULL	NULL	0	NULL	estrogen 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Ovariectomized mice were treated with estrogen and progesterone on a schedule to mimic early pregnancy .
	manualset3
117499	3	404637	5	NULL	NULL	0	NULL	progesterone 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Ovariectomized mice were treated with estrogen and progesterone on a schedule to mimic early pregnancy .
	manualset3
117500	4	404637	5	NULL	NULL	0	NULL	schedule 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ovariectomized mice were treated with estrogen and progesterone on a schedule to mimic early pregnancy .
	manualset3
117501	5	404637	5	NULL	NULL	0	NULL	early pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ovariectomized mice were treated with estrogen and progesterone on a schedule to mimic early pregnancy .
	manualset3
117503	1	404638	5	NULL	NULL	0	NULL	Ovariectomy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ovariectomy decreased D ( 2 ) agonist and antagonist striatal binding sites , specific binding was measured using ( ( 3 ) H ) quinpirole and ( ( 3 ) H ) spiperone .
	manualset3
117507	2	404638	5	NULL	NULL	0	NULL	D ( 2 ) agonist 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Ovariectomy decreased D ( 2 ) agonist and antagonist striatal binding sites , specific binding was measured using ( ( 3 ) H ) quinpirole and ( ( 3 ) H ) spiperone .
	manualset3
117509	3	404638	5	NULL	NULL	0	NULL	antagonist striatal binding sites	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ovariectomy decreased D ( 2 ) agonist and antagonist striatal binding sites , specific binding was measured using ( ( 3 ) H ) quinpirole and ( ( 3 ) H ) spiperone .
	manualset3
117510	4	404638	5	NULL	NULL	0	NULL	 ( ( 3 ) H ) quinpirole	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Ovariectomy decreased D ( 2 ) agonist and antagonist striatal binding sites , specific binding was measured using ( ( 3 ) H ) quinpirole and ( ( 3 ) H ) spiperone .
	manualset3
117538	5	404638	5	NULL	NULL	0	NULL	( ( 3 ) H ) spiperone 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Ovariectomy decreased D ( 2 ) agonist and antagonist striatal binding sites , specific binding was measured using ( ( 3 ) H ) quinpirole and ( ( 3 ) H ) spiperone .
	manualset3
121233	6	404638	5	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ovariectomy decreased D ( 2 ) agonist and antagonist striatal binding sites , specific binding was measured using ( ( 3 ) H ) quinpirole and ( ( 3 ) H ) spiperone .
	manualset3
117539	1	404639	5	NULL	NULL	0	NULL	Ovaries 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ovaries incubated in the presence of VEGF or NRG had no change in follicle development .
	manualset3
117540	2	404639	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ovaries incubated in the presence of VEGF or NRG had no change in follicle development .
	manualset3
117541	3	404639	5	NULL	NULL	0	NULL	VEGF 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Ovaries incubated in the presence of VEGF or NRG had no change in follicle development .
	manualset3
117542	4	404639	5	NULL	NULL	0	NULL	NRG 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Ovaries incubated in the presence of VEGF or NRG had no change in follicle development .
	manualset3
117543	5	404639	5	NULL	NULL	0	NULL	change 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ovaries incubated in the presence of VEGF or NRG had no change in follicle development .
	manualset3
117544	6	404639	5	NULL	NULL	0	NULL	follicle development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ovaries incubated in the presence of VEGF or NRG had no change in follicle development .
	manualset3
117546	1	404640	5	NULL	NULL	0	NULL	150 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 150 systematic reviews relevant to chronic pain treatment were identified and their quality assessed using a simple scoring system .
	manualset3
117547	2	404640	5	NULL	NULL	0	NULL	systematic reviews 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 150 systematic reviews relevant to chronic pain treatment were identified and their quality assessed using a simple scoring system .
	manualset3
117548	3	404640	5	NULL	NULL	0	NULL	chronic pain treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 150 systematic reviews relevant to chronic pain treatment were identified and their quality assessed using a simple scoring system .
	manualset3
117555	4	404640	5	NULL	NULL	0	NULL	quality 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 150 systematic reviews relevant to chronic pain treatment were identified and their quality assessed using a simple scoring system .
	manualset3
117556	5	404640	5	NULL	NULL	0	NULL	simple scoring system 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 150 systematic reviews relevant to chronic pain treatment were identified and their quality assessed using a simple scoring system .
	manualset3
117557	1	404641	5	NULL	NULL	0	NULL	30 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 30 % of the IgG synthesized by 9 of 11 synovia had an isoelectric point greater than 8 ( cathodal shift ) , while 55 % of the synovia secreted IgG showing oligoclonal banding by isoelectric focusing .
	manualset3
117558	2	404641	5	NULL	NULL	0	NULL	IgG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 30 % of the IgG synthesized by 9 of 11 synovia had an isoelectric point greater than 8 ( cathodal shift ) , while 55 % of the synovia secreted IgG showing oligoclonal banding by isoelectric focusing .
	manualset3
117559	3	404641	5	NULL	NULL	0	NULL	9 of 11 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 30 % of the IgG synthesized by 9 of 11 synovia had an isoelectric point greater than 8 ( cathodal shift ) , while 55 % of the synovia secreted IgG showing oligoclonal banding by isoelectric focusing .
	manualset3
117560	4	404641	5	NULL	NULL	0	NULL	synovia 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 30 % of the IgG synthesized by 9 of 11 synovia had an isoelectric point greater than 8 ( cathodal shift ) , while 55 % of the synovia secreted IgG showing oligoclonal banding by isoelectric focusing .
	manualset3
117561	5	404641	5	NULL	NULL	0	NULL	isoelectric point	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 30 % of the IgG synthesized by 9 of 11 synovia had an isoelectric point greater than 8 ( cathodal shift ) , while 55 % of the synovia secreted IgG showing oligoclonal banding by isoelectric focusing .
	manualset3
117562	6	404641	5	NULL	NULL	0	NULL	8	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 30 % of the IgG synthesized by 9 of 11 synovia had an isoelectric point greater than 8 ( cathodal shift ) , while 55 % of the synovia secreted IgG showing oligoclonal banding by isoelectric focusing .
	manualset3
117564	7	404641	5	NULL	NULL	0	NULL	cathodal shift	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 30 % of the IgG synthesized by 9 of 11 synovia had an isoelectric point greater than 8 ( cathodal shift ) , while 55 % of the synovia secreted IgG showing oligoclonal banding by isoelectric focusing .
	manualset3
117566	8	404641	5	NULL	NULL	0	NULL	 55 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 30 % of the IgG synthesized by 9 of 11 synovia had an isoelectric point greater than 8 ( cathodal shift ) , while 55 % of the synovia secreted IgG showing oligoclonal banding by isoelectric focusing .
	manualset3
117567	9	404641	5	NULL	NULL	0	NULL	synovia secreted IgG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 30 % of the IgG synthesized by 9 of 11 synovia had an isoelectric point greater than 8 ( cathodal shift ) , while 55 % of the synovia secreted IgG showing oligoclonal banding by isoelectric focusing .
	manualset3
117568	10	404641	5	NULL	NULL	0	NULL	isoelectric focusing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 30 % of the IgG synthesized by 9 of 11 synovia had an isoelectric point greater than 8 ( cathodal shift ) , while 55 % of the synovia secreted IgG showing oligoclonal banding by isoelectric focusing .
	manualset3
117571	1	404642	5	NULL	NULL	0	NULL	 4 , 000	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 4 , 000 specimens of 4 Culex species in 235 species-specific pools were tested for the presence of West Nile , St. Louis , and western equine encephalitis viruses .
	manualset3
117573	2	404642	5	NULL	NULL	NULL	NULL	specimens 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Over 4 , 000 specimens of 4 Culex species in 235 species-specific pools were tested for the presence of West Nile , St. Louis , and western equine encephalitis viruses .
	manualset3
117575	3	404642	5	NULL	NULL	0	NULL	4	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 4 , 000 specimens of 4 Culex species in 235 species-specific pools were tested for the presence of West Nile , St. Louis , and western equine encephalitis viruses .
	manualset3
117576	4	404642	5	NULL	NULL	0	NULL	Culex species 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 4 , 000 specimens of 4 Culex species in 235 species-specific pools were tested for the presence of West Nile , St. Louis , and western equine encephalitis viruses .
	manualset3
117577	5	404642	5	NULL	NULL	0	NULL	 235 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 4 , 000 specimens of 4 Culex species in 235 species-specific pools were tested for the presence of West Nile , St. Louis , and western equine encephalitis viruses .
	manualset3
117578	6	404642	5	NULL	NULL	0	NULL	species-specific pools	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 4 , 000 specimens of 4 Culex species in 235 species-specific pools were tested for the presence of West Nile , St. Louis , and western equine encephalitis viruses .
	manualset3
117579	7	404642	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 4 , 000 specimens of 4 Culex species in 235 species-specific pools were tested for the presence of West Nile , St. Louis , and western equine encephalitis viruses .
	manualset3
117584	8	404642	5	NULL	NULL	0	NULL	West Nile encephalitis viruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 4 , 000 specimens of 4 Culex species in 235 species-specific pools were tested for the presence of West Nile , St. Louis , and western equine encephalitis viruses .
	manualset3
117585	9	404642	5	NULL	NULL	0	NULL	St. Louis encephalitis viruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 4 , 000 specimens of 4 Culex species in 235 species-specific pools were tested for the presence of West Nile , St. Louis , and western equine encephalitis viruses .
	manualset3
117586	10	404642	5	NULL	NULL	0	NULL	western equine encephalitis viruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 4 , 000 specimens of 4 Culex species in 235 species-specific pools were tested for the presence of West Nile , St. Louis , and western equine encephalitis viruses .
	manualset3
117587	1	404643	5	NULL	NULL	0	NULL	 4 years 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 4 years , we have treated 40 patients ( hyperthyroid ( Plummer 's disease ) : 6 , single hot nodules with undetectable thyrotropin ( TSH ) and normal serum free thyroxine ( FT4 ) : 34 ) , 34 single hot nodules with undetectable thyrotropin TSH and normal serum free thyroxine ( FT4 ) with 131I .
	manualset3
117588	2	404643	5	NULL	NULL	0	NULL	 40 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 4 years , we have treated 40 patients ( hyperthyroid ( Plummer 's disease ) : 6 , single hot nodules with undetectable thyrotropin ( TSH ) and normal serum free thyroxine ( FT4 ) : 34 ) , 34 single hot nodules with undetectable thyrotropin TSH and normal serum free thyroxine ( FT4 ) with 131I .
	manualset3
117589	3	404643	5	NULL	NULL	0	NULL	hyperthyroid ( Plummer 's disease )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 4 years , we have treated 40 patients ( hyperthyroid ( Plummer 's disease ) : 6 , single hot nodules with undetectable thyrotropin ( TSH ) and normal serum free thyroxine ( FT4 ) : 34 ) , 34 single hot nodules with undetectable thyrotropin TSH and normal serum free thyroxine ( FT4 ) with 131I .
	manualset3
117590	4	404643	5	NULL	NULL	0	NULL	6	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 4 years , we have treated 40 patients ( hyperthyroid ( Plummer 's disease ) : 6 , single hot nodules with undetectable thyrotropin ( TSH ) and normal serum free thyroxine ( FT4 ) : 34 ) , 34 single hot nodules with undetectable thyrotropin TSH and normal serum free thyroxine ( FT4 ) with 131I .
	manualset3
117593	5	404643	5	NULL	NULL	0	NULL	single hot nodules with undetectable thyrotropin ( TSH )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 4 years , we have treated 40 patients ( hyperthyroid ( Plummer 's disease ) : 6 , single hot nodules with undetectable thyrotropin ( TSH ) and normal serum free thyroxine ( FT4 ) : 34 ) , 34 single hot nodules with undetectable thyrotropin TSH and normal serum free thyroxine ( FT4 ) with 131I .
	manualset3
117595	6	404643	5	NULL	NULL	0	NULL	single hot nodules with normal serum free thyroxine ( FT4 ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 4 years , we have treated 40 patients ( hyperthyroid ( Plummer 's disease ) : 6 , single hot nodules with undetectable thyrotropin ( TSH ) and normal serum free thyroxine ( FT4 ) : 34 ) , 34 single hot nodules with undetectable thyrotropin TSH and normal serum free thyroxine ( FT4 ) with 131I .
	manualset3
117596	7	404643	5	NULL	NULL	0	NULL	34	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 4 years , we have treated 40 patients ( hyperthyroid ( Plummer 's disease ) : 6 , single hot nodules with undetectable thyrotropin ( TSH ) and normal serum free thyroxine ( FT4 ) : 34 ) , 34 single hot nodules with undetectable thyrotropin TSH and normal serum free thyroxine ( FT4 ) with 131I .
	manualset3
117597	8	404643	5	NULL	NULL	NULL	NULL	34	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Over 4 years , we have treated 40 patients ( hyperthyroid ( Plummer 's disease ) : 6 , single hot nodules with undetectable thyrotropin ( TSH ) and normal serum free thyroxine ( FT4 ) : 34 ) , 34 single hot nodules with undetectable thyrotropin TSH and normal serum free thyroxine ( FT4 ) with 131I .
	manualset3
119167	9	404643	5	NULL	NULL	0	NULL	single hot nodules with undetectable thyrotropin TSH	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 4 years , we have treated 40 patients ( hyperthyroid ( Plummer 's disease ) : 6 , single hot nodules with undetectable thyrotropin ( TSH ) and normal serum free thyroxine ( FT4 ) : 34 ) , 34 single hot nodules with undetectable thyrotropin TSH and normal serum free thyroxine ( FT4 ) with 131I .
	manualset3
119168	10	404643	5	NULL	NULL	0	NULL	single hot nodules with normal serum free thyroxine ( FT4 )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 4 years , we have treated 40 patients ( hyperthyroid ( Plummer 's disease ) : 6 , single hot nodules with undetectable thyrotropin ( TSH ) and normal serum free thyroxine ( FT4 ) : 34 ) , 34 single hot nodules with undetectable thyrotropin TSH and normal serum free thyroxine ( FT4 ) with 131I .
	manualset3
119169	11	404643	5	NULL	NULL	0	NULL	131I	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Over 4 years , we have treated 40 patients ( hyperthyroid ( Plummer 's disease ) : 6 , single hot nodules with undetectable thyrotropin ( TSH ) and normal serum free thyroxine ( FT4 ) : 34 ) , 34 single hot nodules with undetectable thyrotropin TSH and normal serum free thyroxine ( FT4 ) with 131I .
	manualset3
117598	1	404644	5	NULL	NULL	0	NULL	evolutionary time	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Over evolutionary time , chromosomal genes located immediately beside MAT have continually been deleted , truncated , or transposed to other places in the genome in a process that is gradually shortening the distance between MAT and HML .
	manualset3
117599	2	404644	5	NULL	NULL	0	NULL	chromosomal genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Over evolutionary time , chromosomal genes located immediately beside MAT have continually been deleted , truncated , or transposed to other places in the genome in a process that is gradually shortening the distance between MAT and HML .
	manualset3
117600	3	404644	5	NULL	NULL	0	NULL	MAT	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Over evolutionary time , chromosomal genes located immediately beside MAT have continually been deleted , truncated , or transposed to other places in the genome in a process that is gradually shortening the distance between MAT and HML .
	manualset3
117601	4	404644	5	NULL	NULL	0	NULL	places 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Over evolutionary time , chromosomal genes located immediately beside MAT have continually been deleted , truncated , or transposed to other places in the genome in a process that is gradually shortening the distance between MAT and HML .
	manualset3
117603	5	404644	5	NULL	NULL	0	NULL	genome 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Over evolutionary time , chromosomal genes located immediately beside MAT have continually been deleted , truncated , or transposed to other places in the genome in a process that is gradually shortening the distance between MAT and HML .
	manualset3
117604	6	404644	5	NULL	NULL	0	NULL	process 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Over evolutionary time , chromosomal genes located immediately beside MAT have continually been deleted , truncated , or transposed to other places in the genome in a process that is gradually shortening the distance between MAT and HML .
	manualset3
117605	7	404644	5	NULL	NULL	0	NULL	distance 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Over evolutionary time , chromosomal genes located immediately beside MAT have continually been deleted , truncated , or transposed to other places in the genome in a process that is gradually shortening the distance between MAT and HML .
	manualset3
117608	8	404644	5	NULL	NULL	0	NULL	MAT 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Over evolutionary time , chromosomal genes located immediately beside MAT have continually been deleted , truncated , or transposed to other places in the genome in a process that is gradually shortening the distance between MAT and HML .
	manualset3
117612	9	404644	5	NULL	NULL	0	NULL	HML 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Over evolutionary time , chromosomal genes located immediately beside MAT have continually been deleted , truncated , or transposed to other places in the genome in a process that is gradually shortening the distance between MAT and HML .
	manualset3
117614	1	404645	5	NULL	NULL	0	NULL	feeding period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Over the feeding period mean change in subjects ' body weight was -0.165 + / - 0.64 % ( means + / - SEM ) of initial body weight .
	manualset3
117615	2	404645	5	NULL	NULL	0	NULL	mean change	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Over the feeding period mean change in subjects ' body weight was -0.165 + / - 0.64 % ( means + / - SEM ) of initial body weight .
	manualset3
117616	3	404645	5	NULL	NULL	0	NULL	subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Over the feeding period mean change in subjects ' body weight was -0.165 + / - 0.64 % ( means + / - SEM ) of initial body weight .
	manualset3
117617	4	404645	5	NULL	NULL	0	NULL	body weight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Over the feeding period mean change in subjects ' body weight was -0.165 + / - 0.64 % ( means + / - SEM ) of initial body weight .
	manualset3
117618	5	404645	5	NULL	NULL	0	NULL	 -0.165 + / - 0.64 % ( means + / - SEM ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Over the feeding period mean change in subjects ' body weight was -0.165 + / - 0.64 % ( means + / - SEM ) of initial body weight .
	manualset3
117619	6	404645	5	NULL	NULL	0	NULL	initial body weight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Over the feeding period mean change in subjects ' body weight was -0.165 + / - 0.64 % ( means + / - SEM ) of initial body weight .
	manualset3
117620	1	404646	5	NULL	NULL	0	NULL	past decade	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Over the past decade , high-dose chemotherapy followed by autologous bone marrow support ( ABMS ) has been employed with increasing frequency to treat patients with a variety of solid tumors .
	manualset3
117621	2	404646	5	NULL	NULL	0	NULL	high-dose chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Over the past decade , high-dose chemotherapy followed by autologous bone marrow support ( ABMS ) has been employed with increasing frequency to treat patients with a variety of solid tumors .
	manualset3
117625	3	404646	5	NULL	NULL	0	NULL	autologous bone marrow support ( ABMS )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Over the past decade , high-dose chemotherapy followed by autologous bone marrow support ( ABMS ) has been employed with increasing frequency to treat patients with a variety of solid tumors .
	manualset3
117626	4	404646	5	NULL	NULL	0	NULL	frequency 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Over the past decade , high-dose chemotherapy followed by autologous bone marrow support ( ABMS ) has been employed with increasing frequency to treat patients with a variety of solid tumors .
	manualset3
117627	5	404646	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Over the past decade , high-dose chemotherapy followed by autologous bone marrow support ( ABMS ) has been employed with increasing frequency to treat patients with a variety of solid tumors .
	manualset3
117628	6	404646	5	NULL	NULL	0	NULL	variety 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Over the past decade , high-dose chemotherapy followed by autologous bone marrow support ( ABMS ) has been employed with increasing frequency to treat patients with a variety of solid tumors .
	manualset3
117630	7	404646	5	NULL	NULL	0	NULL	solid tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Over the past decade , high-dose chemotherapy followed by autologous bone marrow support ( ABMS ) has been employed with increasing frequency to treat patients with a variety of solid tumors .
	manualset3
117631	1	404647	5	NULL	NULL	0	NULL	past decades	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Over the past decades , genetically engineered mouse models have been used to study hair follicle morphogenesis and significant advances have been made toward the identification of key signaling pathways and the regulatory genes involved .
	manualset3
117632	2	404647	5	NULL	NULL	0	NULL	genetically engineered mouse models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Over the past decades , genetically engineered mouse models have been used to study hair follicle morphogenesis and significant advances have been made toward the identification of key signaling pathways and the regulatory genes involved .
	manualset3
117633	3	404647	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Over the past decades , genetically engineered mouse models have been used to study hair follicle morphogenesis and significant advances have been made toward the identification of key signaling pathways and the regulatory genes involved .
	manualset3
117634	4	404647	5	NULL	NULL	0	NULL	hair follicle morphogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Over the past decades , genetically engineered mouse models have been used to study hair follicle morphogenesis and significant advances have been made toward the identification of key signaling pathways and the regulatory genes involved .
	manualset3
117635	5	404647	5	NULL	NULL	0	NULL	significant advances 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Over the past decades , genetically engineered mouse models have been used to study hair follicle morphogenesis and significant advances have been made toward the identification of key signaling pathways and the regulatory genes involved .
	manualset3
117638	6	404647	5	NULL	NULL	0	NULL	identification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Over the past decades , genetically engineered mouse models have been used to study hair follicle morphogenesis and significant advances have been made toward the identification of key signaling pathways and the regulatory genes involved .
	manualset3
117639	7	404647	5	NULL	NULL	0	NULL	key signaling pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Over the past decades , genetically engineered mouse models have been used to study hair follicle morphogenesis and significant advances have been made toward the identification of key signaling pathways and the regulatory genes involved .
	manualset3
117642	8	404647	5	NULL	NULL	0	NULL	regulatory genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Over the past decades , genetically engineered mouse models have been used to study hair follicle morphogenesis and significant advances have been made toward the identification of key signaling pathways and the regulatory genes involved .
	manualset3
117646	1	404648	5	NULL	NULL	0	NULL	data set	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , our data set together with prior results likely identify the majority of nudivirus-related genes that are transcriptionally functional during BV replication .
	manualset3
117648	2	404648	5	NULL	NULL	0	NULL	prior results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , our data set together with prior results likely identify the majority of nudivirus-related genes that are transcriptionally functional during BV replication .
	manualset3
117650	3	404648	5	NULL	NULL	0	NULL	identify 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , our data set together with prior results likely identify the majority of nudivirus-related genes that are transcriptionally functional during BV replication .
	manualset3
117651	4	404648	5	NULL	NULL	0	NULL	majority 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , our data set together with prior results likely identify the majority of nudivirus-related genes that are transcriptionally functional during BV replication .
	manualset3
117653	5	404648	5	NULL	NULL	0	NULL	nudivirus-related genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , our data set together with prior results likely identify the majority of nudivirus-related genes that are transcriptionally functional during BV replication .
	manualset3
117658	6	404648	5	NULL	NULL	0	NULL	BV replication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , our data set together with prior results likely identify the majority of nudivirus-related genes that are transcriptionally functional during BV replication .
	manualset3
117661	1	404649	5	NULL	NULL	0	NULL	findings 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , our findings suggest that Akt is a key component of anti-apoptotic pathways stimulated by P. gingivalis .
	manualset3
117662	2	404649	5	NULL	NULL	0	NULL	Akt 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , our findings suggest that Akt is a key component of anti-apoptotic pathways stimulated by P. gingivalis .
	manualset3
117663	3	404649	5	NULL	NULL	0	NULL	key component	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , our findings suggest that Akt is a key component of anti-apoptotic pathways stimulated by P. gingivalis .
	manualset3
117664	4	404649	5	NULL	NULL	0	NULL	anti-apoptotic pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , our findings suggest that Akt is a key component of anti-apoptotic pathways stimulated by P. gingivalis .
	manualset3
117665	5	404649	5	NULL	NULL	0	NULL	P. gingivalis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , our findings suggest that Akt is a key component of anti-apoptotic pathways stimulated by P. gingivalis .
	manualset3
117666	1	404650	5	NULL	NULL	0	NULL	DOC uptake	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall DOC uptake at pseudo-steady state differed between the two tested GACs ( 18.9 and 28.6 g-C/kg GAC ) , and the percent difference in DOC uptake closely matched the percent difference in the volume of pores with widths in the 1-50 nm range that was measured for the two fresh GACs .
	manualset3
117673	2	404650	5	NULL	NULL	0	NULL	pseudo-steady state	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall DOC uptake at pseudo-steady state differed between the two tested GACs ( 18.9 and 28.6 g-C/kg GAC ) , and the percent difference in DOC uptake closely matched the percent difference in the volume of pores with widths in the 1-50 nm range that was measured for the two fresh GACs .
	manualset3
117686	3	404650	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall DOC uptake at pseudo-steady state differed between the two tested GACs ( 18.9 and 28.6 g-C/kg GAC ) , and the percent difference in DOC uptake closely matched the percent difference in the volume of pores with widths in the 1-50 nm range that was measured for the two fresh GACs .
	manualset3
117687	4	404650	5	NULL	NULL	0	NULL	GACs 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall DOC uptake at pseudo-steady state differed between the two tested GACs ( 18.9 and 28.6 g-C/kg GAC ) , and the percent difference in DOC uptake closely matched the percent difference in the volume of pores with widths in the 1-50 nm range that was measured for the two fresh GACs .
	manualset3
117688	5	404650	5	NULL	NULL	0	NULL	18.9 g-C/kg GAC	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall DOC uptake at pseudo-steady state differed between the two tested GACs ( 18.9 and 28.6 g-C/kg GAC ) , and the percent difference in DOC uptake closely matched the percent difference in the volume of pores with widths in the 1-50 nm range that was measured for the two fresh GACs .
	manualset3
117689	6	404650	5	NULL	NULL	0	NULL	28.6 g-C/kg GAC 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall DOC uptake at pseudo-steady state differed between the two tested GACs ( 18.9 and 28.6 g-C/kg GAC ) , and the percent difference in DOC uptake closely matched the percent difference in the volume of pores with widths in the 1-50 nm range that was measured for the two fresh GACs .
	manualset3
117690	7	404650	5	NULL	NULL	0	NULL	percent difference	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall DOC uptake at pseudo-steady state differed between the two tested GACs ( 18.9 and 28.6 g-C/kg GAC ) , and the percent difference in DOC uptake closely matched the percent difference in the volume of pores with widths in the 1-50 nm range that was measured for the two fresh GACs .
	manualset3
117691	8	404650	5	NULL	NULL	0	NULL	DOC uptake	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall DOC uptake at pseudo-steady state differed between the two tested GACs ( 18.9 and 28.6 g-C/kg GAC ) , and the percent difference in DOC uptake closely matched the percent difference in the volume of pores with widths in the 1-50 nm range that was measured for the two fresh GACs .
	manualset3
117692	9	404650	5	NULL	NULL	0	NULL	percent difference	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall DOC uptake at pseudo-steady state differed between the two tested GACs ( 18.9 and 28.6 g-C/kg GAC ) , and the percent difference in DOC uptake closely matched the percent difference in the volume of pores with widths in the 1-50 nm range that was measured for the two fresh GACs .
	manualset3
117693	10	404650	5	NULL	NULL	0	NULL	volume 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall DOC uptake at pseudo-steady state differed between the two tested GACs ( 18.9 and 28.6 g-C/kg GAC ) , and the percent difference in DOC uptake closely matched the percent difference in the volume of pores with widths in the 1-50 nm range that was measured for the two fresh GACs .
	manualset3
117694	11	404650	5	NULL	NULL	0	NULL	pores 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall DOC uptake at pseudo-steady state differed between the two tested GACs ( 18.9 and 28.6 g-C/kg GAC ) , and the percent difference in DOC uptake closely matched the percent difference in the volume of pores with widths in the 1-50 nm range that was measured for the two fresh GACs .
	manualset3
117695	12	404650	5	NULL	NULL	0	NULL	widths 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall DOC uptake at pseudo-steady state differed between the two tested GACs ( 18.9 and 28.6 g-C/kg GAC ) , and the percent difference in DOC uptake closely matched the percent difference in the volume of pores with widths in the 1-50 nm range that was measured for the two fresh GACs .
	manualset3
117696	13	404650	5	NULL	NULL	0	NULL	 1-50 nm range	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall DOC uptake at pseudo-steady state differed between the two tested GACs ( 18.9 and 28.6 g-C/kg GAC ) , and the percent difference in DOC uptake closely matched the percent difference in the volume of pores with widths in the 1-50 nm range that was measured for the two fresh GACs .
	manualset3
117697	14	404650	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall DOC uptake at pseudo-steady state differed between the two tested GACs ( 18.9 and 28.6 g-C/kg GAC ) , and the percent difference in DOC uptake closely matched the percent difference in the volume of pores with widths in the 1-50 nm range that was measured for the two fresh GACs .
	manualset3
117698	15	404650	5	NULL	NULL	0	NULL	fresh GACs	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall DOC uptake at pseudo-steady state differed between the two tested GACs ( 18.9 and 28.6 g-C/kg GAC ) , and the percent difference in DOC uptake closely matched the percent difference in the volume of pores with widths in the 1-50 nm range that was measured for the two fresh GACs .
	manualset3
117699	1	404651	5	NULL	NULL	0	NULL	Overall accuracies 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall accuracies for both operated and clinical groups was ultrasound 57 % , gallium 54 % , and CT 67 % , not significantly different results .
	manualset3
117700	2	404651	5	NULL	NULL	0	NULL	operated group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall accuracies for both operated and clinical groups was ultrasound 57 % , gallium 54 % , and CT 67 % , not significantly different results .
	manualset3
117701	3	404651	5	NULL	NULL	0	NULL	clinical groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall accuracies for both operated and clinical groups was ultrasound 57 % , gallium 54 % , and CT 67 % , not significantly different results .
	manualset3
117702	4	404651	5	NULL	NULL	0	NULL	ultrasound 57 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall accuracies for both operated and clinical groups was ultrasound 57 % , gallium 54 % , and CT 67 % , not significantly different results .
	manualset3
117703	5	404651	5	NULL	NULL	0	NULL	gallium 54 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall accuracies for both operated and clinical groups was ultrasound 57 % , gallium 54 % , and CT 67 % , not significantly different results .
	manualset3
117704	6	404651	5	NULL	NULL	0	NULL	CT 67 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall accuracies for both operated and clinical groups was ultrasound 57 % , gallium 54 % , and CT 67 % , not significantly different results .
	manualset3
117705	1	404652	5	NULL	NULL	0	NULL	Overall rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall rates of childhood anxiety disorders are estimated to be from 6 % to 10 % , depending upon categories included and strategies for ascertainment .
	manualset3
117706	2	404652	5	NULL	NULL	0	NULL	childhood anxiety disorders 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall rates of childhood anxiety disorders are estimated to be from 6 % to 10 % , depending upon categories included and strategies for ascertainment .
	manualset3
117707	3	404652	5	NULL	NULL	0	NULL	 6 % to 10 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall rates of childhood anxiety disorders are estimated to be from 6 % to 10 % , depending upon categories included and strategies for ascertainment .
	manualset3
117708	4	404652	5	NULL	NULL	0	NULL	categories 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall rates of childhood anxiety disorders are estimated to be from 6 % to 10 % , depending upon categories included and strategies for ascertainment .
	manualset3
117709	5	404652	5	NULL	NULL	0	NULL	strategies 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall rates of childhood anxiety disorders are estimated to be from 6 % to 10 % , depending upon categories included and strategies for ascertainment .
	manualset3
117710	6	404652	5	NULL	NULL	0	NULL	ascertainment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall rates of childhood anxiety disorders are estimated to be from 6 % to 10 % , depending upon categories included and strategies for ascertainment .
	manualset3
117711	1	404653	5	NULL	NULL	0	NULL	Overall sequence comparison	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall sequence comparison shows high identity to both trout NCX-TR1 .0 ( approximately 81 % ) and mammalian NCX1 .1 ( approximately 73 % ) , and phylogenetic analyses confirmed its identity as a member of the NCX1 gene family , expressing exons A , C , D , and F in the alternative splice site .
	manualset3
117712	2	404653	5	NULL	NULL	0	NULL	high identity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall sequence comparison shows high identity to both trout NCX-TR1 .0 ( approximately 81 % ) and mammalian NCX1 .1 ( approximately 73 % ) , and phylogenetic analyses confirmed its identity as a member of the NCX1 gene family , expressing exons A , C , D , and F in the alternative splice site .
	manualset3
118018	3	404653	5	NULL	NULL	NULL	NULL	trout NCX-TR1 .0	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Overall sequence comparison shows high identity to both trout NCX-TR1 .0 ( approximately 81 % ) and mammalian NCX1 .1 ( approximately 73 % ) , and phylogenetic analyses confirmed its identity as a member of the NCX1 gene family , expressing exons A , C , D , and F in the alternative splice site .
	manualset3
118019	4	404653	5	NULL	NULL	0	NULL	81 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall sequence comparison shows high identity to both trout NCX-TR1 .0 ( approximately 81 % ) and mammalian NCX1 .1 ( approximately 73 % ) , and phylogenetic analyses confirmed its identity as a member of the NCX1 gene family , expressing exons A , C , D , and F in the alternative splice site .
	manualset3
118020	5	404653	5	NULL	NULL	NULL	NULL	mammalian NCX1 .1	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Overall sequence comparison shows high identity to both trout NCX-TR1 .0 ( approximately 81 % ) and mammalian NCX1 .1 ( approximately 73 % ) , and phylogenetic analyses confirmed its identity as a member of the NCX1 gene family , expressing exons A , C , D , and F in the alternative splice site .
	manualset3
118021	6	404653	5	NULL	NULL	0	NULL	73 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall sequence comparison shows high identity to both trout NCX-TR1 .0 ( approximately 81 % ) and mammalian NCX1 .1 ( approximately 73 % ) , and phylogenetic analyses confirmed its identity as a member of the NCX1 gene family , expressing exons A , C , D , and F in the alternative splice site .
	manualset3
118022	7	404653	5	NULL	NULL	0	NULL	phylogenetic analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall sequence comparison shows high identity to both trout NCX-TR1 .0 ( approximately 81 % ) and mammalian NCX1 .1 ( approximately 73 % ) , and phylogenetic analyses confirmed its identity as a member of the NCX1 gene family , expressing exons A , C , D , and F in the alternative splice site .
	manualset3
118023	8	404653	5	NULL	NULL	0	NULL	identity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall sequence comparison shows high identity to both trout NCX-TR1 .0 ( approximately 81 % ) and mammalian NCX1 .1 ( approximately 73 % ) , and phylogenetic analyses confirmed its identity as a member of the NCX1 gene family , expressing exons A , C , D , and F in the alternative splice site .
	manualset3
118024	9	404653	5	NULL	NULL	0	NULL	member 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall sequence comparison shows high identity to both trout NCX-TR1 .0 ( approximately 81 % ) and mammalian NCX1 .1 ( approximately 73 % ) , and phylogenetic analyses confirmed its identity as a member of the NCX1 gene family , expressing exons A , C , D , and F in the alternative splice site .
	manualset3
118025	10	404653	5	NULL	NULL	0	NULL	NCX1 gene family 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall sequence comparison shows high identity to both trout NCX-TR1 .0 ( approximately 81 % ) and mammalian NCX1 .1 ( approximately 73 % ) , and phylogenetic analyses confirmed its identity as a member of the NCX1 gene family , expressing exons A , C , D , and F in the alternative splice site .
	manualset3
118026	11	404653	5	NULL	NULL	0	NULL	exon A 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall sequence comparison shows high identity to both trout NCX-TR1 .0 ( approximately 81 % ) and mammalian NCX1 .1 ( approximately 73 % ) , and phylogenetic analyses confirmed its identity as a member of the NCX1 gene family , expressing exons A , C , D , and F in the alternative splice site .
	manualset3
118027	12	404653	5	NULL	NULL	0	NULL	exon C 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall sequence comparison shows high identity to both trout NCX-TR1 .0 ( approximately 81 % ) and mammalian NCX1 .1 ( approximately 73 % ) , and phylogenetic analyses confirmed its identity as a member of the NCX1 gene family , expressing exons A , C , D , and F in the alternative splice site .
	manualset3
118028	13	404653	5	NULL	NULL	0	NULL	exon D	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall sequence comparison shows high identity to both trout NCX-TR1 .0 ( approximately 81 % ) and mammalian NCX1 .1 ( approximately 73 % ) , and phylogenetic analyses confirmed its identity as a member of the NCX1 gene family , expressing exons A , C , D , and F in the alternative splice site .
	manualset3
118029	14	404653	5	NULL	NULL	0	NULL	exon F	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall sequence comparison shows high identity to both trout NCX-TR1 .0 ( approximately 81 % ) and mammalian NCX1 .1 ( approximately 73 % ) , and phylogenetic analyses confirmed its identity as a member of the NCX1 gene family , expressing exons A , C , D , and F in the alternative splice site .
	manualset3
118030	15	404653	5	NULL	NULL	0	NULL	alternative splice site	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall sequence comparison shows high identity to both trout NCX-TR1 .0 ( approximately 81 % ) and mammalian NCX1 .1 ( approximately 73 % ) , and phylogenetic analyses confirmed its identity as a member of the NCX1 gene family , expressing exons A , C , D , and F in the alternative splice site .
	manualset3
118031	1	404654	5	NULL	NULL	0	NULL	88.5 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , 88.5 % of the paired Etest results for amphotericin B agreed to within two concentrations , as did 94 % of results for flucytosine , 92 % for fluconazole and 79 % for itraconazole .
	manualset3
118032	2	404654	5	NULL	NULL	0	NULL	 Etest results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , 88.5 % of the paired Etest results for amphotericin B agreed to within two concentrations , as did 94 % of results for flucytosine , 92 % for fluconazole and 79 % for itraconazole .
	manualset3
118033	3	404654	5	NULL	NULL	0	NULL	amphotericin B	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , 88.5 % of the paired Etest results for amphotericin B agreed to within two concentrations , as did 94 % of results for flucytosine , 92 % for fluconazole and 79 % for itraconazole .
	manualset3
118034	4	404654	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , 88.5 % of the paired Etest results for amphotericin B agreed to within two concentrations , as did 94 % of results for flucytosine , 92 % for fluconazole and 79 % for itraconazole .
	manualset3
118035	5	404654	5	NULL	NULL	0	NULL	concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , 88.5 % of the paired Etest results for amphotericin B agreed to within two concentrations , as did 94 % of results for flucytosine , 92 % for fluconazole and 79 % for itraconazole .
	manualset3
118036	6	404654	5	NULL	NULL	0	NULL	94 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , 88.5 % of the paired Etest results for amphotericin B agreed to within two concentrations , as did 94 % of results for flucytosine , 92 % for fluconazole and 79 % for itraconazole .
	manualset3
118037	7	404654	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , 88.5 % of the paired Etest results for amphotericin B agreed to within two concentrations , as did 94 % of results for flucytosine , 92 % for fluconazole and 79 % for itraconazole .
	manualset3
118038	8	404654	5	NULL	NULL	0	NULL	flucytosine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , 88.5 % of the paired Etest results for amphotericin B agreed to within two concentrations , as did 94 % of results for flucytosine , 92 % for fluconazole and 79 % for itraconazole .
	manualset3
118039	9	404654	5	NULL	NULL	0	NULL	92 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , 88.5 % of the paired Etest results for amphotericin B agreed to within two concentrations , as did 94 % of results for flucytosine , 92 % for fluconazole and 79 % for itraconazole .
	manualset3
118040	10	404654	5	NULL	NULL	0	NULL	fluconazole 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , 88.5 % of the paired Etest results for amphotericin B agreed to within two concentrations , as did 94 % of results for flucytosine , 92 % for fluconazole and 79 % for itraconazole .
	manualset3
118041	11	404654	5	NULL	NULL	0	NULL	 79 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , 88.5 % of the paired Etest results for amphotericin B agreed to within two concentrations , as did 94 % of results for flucytosine , 92 % for fluconazole and 79 % for itraconazole .
	manualset3
118042	12	404654	5	NULL	NULL	0	NULL	itraconazole 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , 88.5 % of the paired Etest results for amphotericin B agreed to within two concentrations , as did 94 % of results for flucytosine , 92 % for fluconazole and 79 % for itraconazole .
	manualset3
118043	1	404655	5	NULL	NULL	0	NULL	California 's public utilities	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , California 's public utilities appear more proactive and target-oriented in asking their customers to conserve than their private counterparts and the state continues to be important in legitimating and guiding conservation behavior , whether the utility is in public hands or private .
	manualset3
118044	2	404655	5	NULL	NULL	0	NULL	customers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , California 's public utilities appear more proactive and target-oriented in asking their customers to conserve than their private counterparts and the state continues to be important in legitimating and guiding conservation behavior , whether the utility is in public hands or private .
	manualset3
118045	3	404655	5	NULL	NULL	0	NULL	private counterparts	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , California 's public utilities appear more proactive and target-oriented in asking their customers to conserve than their private counterparts and the state continues to be important in legitimating and guiding conservation behavior , whether the utility is in public hands or private .
	manualset3
118046	4	404655	5	NULL	NULL	0	NULL	state 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , California 's public utilities appear more proactive and target-oriented in asking their customers to conserve than their private counterparts and the state continues to be important in legitimating and guiding conservation behavior , whether the utility is in public hands or private .
	manualset3
118047	5	404655	5	NULL	NULL	0	NULL	conservation behavior	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , California 's public utilities appear more proactive and target-oriented in asking their customers to conserve than their private counterparts and the state continues to be important in legitimating and guiding conservation behavior , whether the utility is in public hands or private .
	manualset3
118048	6	404655	5	NULL	NULL	0	NULL	utility 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , California 's public utilities appear more proactive and target-oriented in asking their customers to conserve than their private counterparts and the state continues to be important in legitimating and guiding conservation behavior , whether the utility is in public hands or private .
	manualset3
118049	7	404655	5	NULL	NULL	0	NULL	public hands	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , California 's public utilities appear more proactive and target-oriented in asking their customers to conserve than their private counterparts and the state continues to be important in legitimating and guiding conservation behavior , whether the utility is in public hands or private .
	manualset3
118050	8	404655	5	NULL	NULL	0	NULL	private 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , California 's public utilities appear more proactive and target-oriented in asking their customers to conserve than their private counterparts and the state continues to be important in legitimating and guiding conservation behavior , whether the utility is in public hands or private .
	manualset3
118106	1	404656	5	NULL	NULL	0	NULL	Fibrotest 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , Fibrotest had the best performance in NALT group , as showed by AUROC of 0.70 and 73.5 % accuracy .
	manualset3
118107	2	404656	5	NULL	NULL	0	NULL	performance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , Fibrotest had the best performance in NALT group , as showed by AUROC of 0.70 and 73.5 % accuracy .
	manualset3
118108	3	404656	5	NULL	NULL	0	NULL	NALT group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , Fibrotest had the best performance in NALT group , as showed by AUROC of 0.70 and 73.5 % accuracy .
	manualset3
118109	4	404656	5	NULL	NULL	0	NULL	AUROC 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , Fibrotest had the best performance in NALT group , as showed by AUROC of 0.70 and 73.5 % accuracy .
	manualset3
118110	5	404656	5	NULL	NULL	0	NULL	0.70 % accuracy 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , Fibrotest had the best performance in NALT group , as showed by AUROC of 0.70 and 73.5 % accuracy .
	manualset3
118111	6	404656	5	NULL	NULL	0	NULL	73.5 % accuracy 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , Fibrotest had the best performance in NALT group , as showed by AUROC of 0.70 and 73.5 % accuracy .
	manualset3
118112	1	404657	5	NULL	NULL	0	NULL	few subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A few subjects had a larger skin reaction to tuberculin than the baseline reading during the 2 to 5 weeks after rash onset .
	manualset3
118113	2	404657	5	NULL	NULL	0	NULL	larger skin reaction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A few subjects had a larger skin reaction to tuberculin than the baseline reading during the 2 to 5 weeks after rash onset .
	manualset3
118114	3	404657	5	NULL	NULL	0	NULL	tuberculin 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A few subjects had a larger skin reaction to tuberculin than the baseline reading during the 2 to 5 weeks after rash onset .
	manualset3
118115	4	404657	5	NULL	NULL	0	NULL	baseline reading	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A few subjects had a larger skin reaction to tuberculin than the baseline reading during the 2 to 5 weeks after rash onset .
	manualset3
118116	5	404657	5	NULL	NULL	0	NULL	2 to 5 weeks 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A few subjects had a larger skin reaction to tuberculin than the baseline reading during the 2 to 5 weeks after rash onset .
	manualset3
118117	6	404657	5	NULL	NULL	0	NULL	rash onset	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A few subjects had a larger skin reaction to tuberculin than the baseline reading during the 2 to 5 weeks after rash onset .
	manualset3
118118	1	404658	5	NULL	NULL	0	NULL	Gram-positive bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , Gram-positive bacteria comprised 72 % ( 1627/2248 ) of recovered isolates and Gram-negative bacteria comprised 28 % ( 621/2248 ) .
	manualset3
118119	2	404658	5	NULL	NULL	0	NULL	72 % ( 1627/2248 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , Gram-positive bacteria comprised 72 % ( 1627/2248 ) of recovered isolates and Gram-negative bacteria comprised 28 % ( 621/2248 ) .
	manualset3
118120	3	404658	5	NULL	NULL	0	NULL	recovered isolates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , Gram-positive bacteria comprised 72 % ( 1627/2248 ) of recovered isolates and Gram-negative bacteria comprised 28 % ( 621/2248 ) .
	manualset3
118121	4	404658	5	NULL	NULL	0	NULL	Gram-negative bacteria 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , Gram-positive bacteria comprised 72 % ( 1627/2248 ) of recovered isolates and Gram-negative bacteria comprised 28 % ( 621/2248 ) .
	manualset3
118122	5	404658	5	NULL	NULL	0	NULL	28 % ( 621/2248 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , Gram-positive bacteria comprised 72 % ( 1627/2248 ) of recovered isolates and Gram-negative bacteria comprised 28 % ( 621/2248 ) .
	manualset3
118123	1	404659	5	NULL	NULL	0	NULL	36 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , about 36 % of the children reported symptoms of atopic disorders .
	manualset3
118124	2	404659	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , about 36 % of the children reported symptoms of atopic disorders .
	manualset3
118125	3	404659	5	NULL	NULL	0	NULL	symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , about 36 % of the children reported symptoms of atopic disorders .
	manualset3
118126	4	404659	5	NULL	NULL	0	NULL	atopic disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , about 36 % of the children reported symptoms of atopic disorders .
	manualset3
118127	1	404660	5	NULL	NULL	0	NULL	bacterial outcomes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , bacterial outcomes were reported in 17 studies , and prevalence of antimicrobial resistance ( AMR ) and multidrug resistance ( MDR ) of zoonotic or potentially zoonotic bacteria in 12 and 7 studies , respectively .
	manualset3
118128	2	404660	5	NULL	NULL	0	NULL	 17 studies	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , bacterial outcomes were reported in 17 studies , and prevalence of antimicrobial resistance ( AMR ) and multidrug resistance ( MDR ) of zoonotic or potentially zoonotic bacteria in 12 and 7 studies , respectively .
	manualset3
118129	3	404660	5	NULL	NULL	0	NULL	prevalence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , bacterial outcomes were reported in 17 studies , and prevalence of antimicrobial resistance ( AMR ) and multidrug resistance ( MDR ) of zoonotic or potentially zoonotic bacteria in 12 and 7 studies , respectively .
	manualset3
118130	4	404660	5	NULL	NULL	0	NULL	antimicrobial resistance ( AMR )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , bacterial outcomes were reported in 17 studies , and prevalence of antimicrobial resistance ( AMR ) and multidrug resistance ( MDR ) of zoonotic or potentially zoonotic bacteria in 12 and 7 studies , respectively .
	manualset3
118131	5	404660	5	NULL	NULL	0	NULL	multidrug resistance ( MDR ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , bacterial outcomes were reported in 17 studies , and prevalence of antimicrobial resistance ( AMR ) and multidrug resistance ( MDR ) of zoonotic or potentially zoonotic bacteria in 12 and 7 studies , respectively .
	manualset3
118132	6	404660	5	NULL	NULL	0	NULL	zoonotic bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , bacterial outcomes were reported in 17 studies , and prevalence of antimicrobial resistance ( AMR ) and multidrug resistance ( MDR ) of zoonotic or potentially zoonotic bacteria in 12 and 7 studies , respectively .
	manualset3
118133	7	404660	5	NULL	NULL	0	NULL	potentially zoonotic bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , bacterial outcomes were reported in 17 studies , and prevalence of antimicrobial resistance ( AMR ) and multidrug resistance ( MDR ) of zoonotic or potentially zoonotic bacteria in 12 and 7 studies , respectively .
	manualset3
118134	8	404660	5	NULL	NULL	0	NULL	12 and 7 studies	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , bacterial outcomes were reported in 17 studies , and prevalence of antimicrobial resistance ( AMR ) and multidrug resistance ( MDR ) of zoonotic or potentially zoonotic bacteria in 12 and 7 studies , respectively .
	manualset3
118135	1	404661	5	NULL	NULL	0	NULL	infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , infection of fetuses with an attenuated virus shows the same immune dysregulation seen postnatally in wild type infected isolator piglets , indicating that : ( a ) attenuation did not alter the ability of the virus to cause dysregulation and ( b ) the isolator infectious model reflects the fetal disease .
	manualset3
118136	2	404661	5	NULL	NULL	0	NULL	fetuses 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , infection of fetuses with an attenuated virus shows the same immune dysregulation seen postnatally in wild type infected isolator piglets , indicating that : ( a ) attenuation did not alter the ability of the virus to cause dysregulation and ( b ) the isolator infectious model reflects the fetal disease .
	manualset3
118137	3	404661	5	NULL	NULL	0	NULL	attenuated virus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , infection of fetuses with an attenuated virus shows the same immune dysregulation seen postnatally in wild type infected isolator piglets , indicating that : ( a ) attenuation did not alter the ability of the virus to cause dysregulation and ( b ) the isolator infectious model reflects the fetal disease .
	manualset3
118138	4	404661	5	NULL	NULL	0	NULL	immune dysregulation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , infection of fetuses with an attenuated virus shows the same immune dysregulation seen postnatally in wild type infected isolator piglets , indicating that : ( a ) attenuation did not alter the ability of the virus to cause dysregulation and ( b ) the isolator infectious model reflects the fetal disease .
	manualset3
118139	5	404661	5	NULL	NULL	0	NULL	wild type infected isolator piglets	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , infection of fetuses with an attenuated virus shows the same immune dysregulation seen postnatally in wild type infected isolator piglets , indicating that : ( a ) attenuation did not alter the ability of the virus to cause dysregulation and ( b ) the isolator infectious model reflects the fetal disease .
	manualset3
118140	6	404661	5	NULL	NULL	0	NULL	attenuation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , infection of fetuses with an attenuated virus shows the same immune dysregulation seen postnatally in wild type infected isolator piglets , indicating that : ( a ) attenuation did not alter the ability of the virus to cause dysregulation and ( b ) the isolator infectious model reflects the fetal disease .
	manualset3
118141	7	404661	5	NULL	NULL	0	NULL	ability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , infection of fetuses with an attenuated virus shows the same immune dysregulation seen postnatally in wild type infected isolator piglets , indicating that : ( a ) attenuation did not alter the ability of the virus to cause dysregulation and ( b ) the isolator infectious model reflects the fetal disease .
	manualset3
118142	8	404661	5	NULL	NULL	0	NULL	virus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , infection of fetuses with an attenuated virus shows the same immune dysregulation seen postnatally in wild type infected isolator piglets , indicating that : ( a ) attenuation did not alter the ability of the virus to cause dysregulation and ( b ) the isolator infectious model reflects the fetal disease .
	manualset3
118143	9	404661	5	NULL	NULL	0	NULL	dysregulation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , infection of fetuses with an attenuated virus shows the same immune dysregulation seen postnatally in wild type infected isolator piglets , indicating that : ( a ) attenuation did not alter the ability of the virus to cause dysregulation and ( b ) the isolator infectious model reflects the fetal disease .
	manualset3
118144	10	404661	5	NULL	NULL	0	NULL	isolator infectious model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , infection of fetuses with an attenuated virus shows the same immune dysregulation seen postnatally in wild type infected isolator piglets , indicating that : ( a ) attenuation did not alter the ability of the virus to cause dysregulation and ( b ) the isolator infectious model reflects the fetal disease .
	manualset3
118145	11	404661	5	NULL	NULL	0	NULL	fetal disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , infection of fetuses with an attenuated virus shows the same immune dysregulation seen postnatally in wild type infected isolator piglets , indicating that : ( a ) attenuation did not alter the ability of the virus to cause dysregulation and ( b ) the isolator infectious model reflects the fetal disease .
	manualset3
118146	1	404662	5	NULL	NULL	0	NULL	macroalgal cover	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , macroalgal cover was negatively related to the cover of live coral and the density of juvenile corals , but displayed no relationship with herbivorous fish biomass .
	manualset3
118147	2	404662	5	NULL	NULL	0	NULL	cover 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , macroalgal cover was negatively related to the cover of live coral and the density of juvenile corals , but displayed no relationship with herbivorous fish biomass .
	manualset3
118148	3	404662	5	NULL	NULL	0	NULL	live coral	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , macroalgal cover was negatively related to the cover of live coral and the density of juvenile corals , but displayed no relationship with herbivorous fish biomass .
	manualset3
118149	4	404662	5	NULL	NULL	0	NULL	density 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , macroalgal cover was negatively related to the cover of live coral and the density of juvenile corals , but displayed no relationship with herbivorous fish biomass .
	manualset3
118150	5	404662	5	NULL	NULL	0	NULL	juvenile corals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , macroalgal cover was negatively related to the cover of live coral and the density of juvenile corals , but displayed no relationship with herbivorous fish biomass .
	manualset3
118151	6	404662	5	NULL	NULL	0	NULL	relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , macroalgal cover was negatively related to the cover of live coral and the density of juvenile corals , but displayed no relationship with herbivorous fish biomass .
	manualset3
118152	7	404662	5	NULL	NULL	NULL	NULL	herbivorous fish biomass	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Overall , macroalgal cover was negatively related to the cover of live coral and the density of juvenile corals , but displayed no relationship with herbivorous fish biomass .
	manualset3
118153	1	404663	5	NULL	NULL	0	NULL	host plant specificity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , no host plant specificity was shown , the three host plant species sharing common bradyrhizobial genotypes that represented 62 % of the collection .
	manualset3
118154	2	404663	5	NULL	NULL	0	NULL	three 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , no host plant specificity was shown , the three host plant species sharing common bradyrhizobial genotypes that represented 62 % of the collection .
	manualset3
118155	3	404663	5	NULL	NULL	0	NULL	host plant species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , no host plant specificity was shown , the three host plant species sharing common bradyrhizobial genotypes that represented 62 % of the collection .
	manualset3
118156	4	404663	5	NULL	NULL	NULL	NULL	bradyrhizobial genotypes 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Overall , no host plant specificity was shown , the three host plant species sharing common bradyrhizobial genotypes that represented 62 % of the collection .
	manualset3
118157	5	404663	5	NULL	NULL	0	NULL	 62 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , no host plant specificity was shown , the three host plant species sharing common bradyrhizobial genotypes that represented 62 % of the collection .
	manualset3
118158	6	404663	5	NULL	NULL	0	NULL	collection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , no host plant specificity was shown , the three host plant species sharing common bradyrhizobial genotypes that represented 62 % of the collection .
	manualset3
118159	1	404664	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , results gathered in this study point to the conclusion that the studied NSAIDs inhibit PLA ( 2 ) activity due to a disturbance of the enzyme binding efficiency to membrane interface possibly by a shielding effect of the Trp residues required for the membrane interfacial binding step that precedes lipolysis process .
	manualset3
118160	2	404664	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , results gathered in this study point to the conclusion that the studied NSAIDs inhibit PLA ( 2 ) activity due to a disturbance of the enzyme binding efficiency to membrane interface possibly by a shielding effect of the Trp residues required for the membrane interfacial binding step that precedes lipolysis process .
	manualset3
118161	3	404664	5	NULL	NULL	0	NULL	conclusion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , results gathered in this study point to the conclusion that the studied NSAIDs inhibit PLA ( 2 ) activity due to a disturbance of the enzyme binding efficiency to membrane interface possibly by a shielding effect of the Trp residues required for the membrane interfacial binding step that precedes lipolysis process .
	manualset3
118162	4	404664	5	NULL	NULL	0	NULL	NSAIDs 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , results gathered in this study point to the conclusion that the studied NSAIDs inhibit PLA ( 2 ) activity due to a disturbance of the enzyme binding efficiency to membrane interface possibly by a shielding effect of the Trp residues required for the membrane interfacial binding step that precedes lipolysis process .
	manualset3
118163	5	404664	5	NULL	NULL	0	NULL	PLA ( 2 ) activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , results gathered in this study point to the conclusion that the studied NSAIDs inhibit PLA ( 2 ) activity due to a disturbance of the enzyme binding efficiency to membrane interface possibly by a shielding effect of the Trp residues required for the membrane interfacial binding step that precedes lipolysis process .
	manualset3
118164	6	404664	5	NULL	NULL	0	NULL	disturbance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , results gathered in this study point to the conclusion that the studied NSAIDs inhibit PLA ( 2 ) activity due to a disturbance of the enzyme binding efficiency to membrane interface possibly by a shielding effect of the Trp residues required for the membrane interfacial binding step that precedes lipolysis process .
	manualset3
118165	7	404664	5	NULL	NULL	0	NULL	enzyme binding efficiency	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , results gathered in this study point to the conclusion that the studied NSAIDs inhibit PLA ( 2 ) activity due to a disturbance of the enzyme binding efficiency to membrane interface possibly by a shielding effect of the Trp residues required for the membrane interfacial binding step that precedes lipolysis process .
	manualset3
118166	8	404664	5	NULL	NULL	0	NULL	membrane interface	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , results gathered in this study point to the conclusion that the studied NSAIDs inhibit PLA ( 2 ) activity due to a disturbance of the enzyme binding efficiency to membrane interface possibly by a shielding effect of the Trp residues required for the membrane interfacial binding step that precedes lipolysis process .
	manualset3
118167	9	404664	5	NULL	NULL	0	NULL	shielding effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , results gathered in this study point to the conclusion that the studied NSAIDs inhibit PLA ( 2 ) activity due to a disturbance of the enzyme binding efficiency to membrane interface possibly by a shielding effect of the Trp residues required for the membrane interfacial binding step that precedes lipolysis process .
	manualset3
118168	10	404664	5	NULL	NULL	0	NULL	Trp residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , results gathered in this study point to the conclusion that the studied NSAIDs inhibit PLA ( 2 ) activity due to a disturbance of the enzyme binding efficiency to membrane interface possibly by a shielding effect of the Trp residues required for the membrane interfacial binding step that precedes lipolysis process .
	manualset3
118169	11	404664	5	NULL	NULL	0	NULL	membrane interfacial binding step	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , results gathered in this study point to the conclusion that the studied NSAIDs inhibit PLA ( 2 ) activity due to a disturbance of the enzyme binding efficiency to membrane interface possibly by a shielding effect of the Trp residues required for the membrane interfacial binding step that precedes lipolysis process .
	manualset3
118170	12	404664	5	NULL	NULL	0	NULL	lipolysis process	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , results gathered in this study point to the conclusion that the studied NSAIDs inhibit PLA ( 2 ) activity due to a disturbance of the enzyme binding efficiency to membrane interface possibly by a shielding effect of the Trp residues required for the membrane interfacial binding step that precedes lipolysis process .
	manualset3
118171	1	404665	5	NULL	NULL	0	NULL	 NEXAFS spectra	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the NEXAFS spectra of water-dispersible soil colloids were similar to the NEXAFS spectrum of the humic acid fraction , but differed clearly from the fulvic acid and dissolved organic matter fractions extracted from the same soil horizon using conventional techniques .
	manualset3
118172	2	404665	5	NULL	NULL	0	NULL	water-dispersible soil colloids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the NEXAFS spectra of water-dispersible soil colloids were similar to the NEXAFS spectrum of the humic acid fraction , but differed clearly from the fulvic acid and dissolved organic matter fractions extracted from the same soil horizon using conventional techniques .
	manualset3
118173	3	404665	5	NULL	NULL	0	NULL	NEXAFS spectrum	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the NEXAFS spectra of water-dispersible soil colloids were similar to the NEXAFS spectrum of the humic acid fraction , but differed clearly from the fulvic acid and dissolved organic matter fractions extracted from the same soil horizon using conventional techniques .
	manualset3
118174	4	404665	5	NULL	NULL	0	NULL	humic acid fraction	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the NEXAFS spectra of water-dispersible soil colloids were similar to the NEXAFS spectrum of the humic acid fraction , but differed clearly from the fulvic acid and dissolved organic matter fractions extracted from the same soil horizon using conventional techniques .
	manualset3
118175	5	404665	5	NULL	NULL	0	NULL	fulvic acid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the NEXAFS spectra of water-dispersible soil colloids were similar to the NEXAFS spectrum of the humic acid fraction , but differed clearly from the fulvic acid and dissolved organic matter fractions extracted from the same soil horizon using conventional techniques .
	manualset3
118176	6	404665	5	NULL	NULL	NULL	NULL	dissolved organic matter fractions	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Overall , the NEXAFS spectra of water-dispersible soil colloids were similar to the NEXAFS spectrum of the humic acid fraction , but differed clearly from the fulvic acid and dissolved organic matter fractions extracted from the same soil horizon using conventional techniques .
	manualset3
118177	7	404665	5	NULL	NULL	0	NULL	soil horizon	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the NEXAFS spectra of water-dispersible soil colloids were similar to the NEXAFS spectrum of the humic acid fraction , but differed clearly from the fulvic acid and dissolved organic matter fractions extracted from the same soil horizon using conventional techniques .
	manualset3
118178	8	404665	5	NULL	NULL	0	NULL	conventional techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the NEXAFS spectra of water-dispersible soil colloids were similar to the NEXAFS spectrum of the humic acid fraction , but differed clearly from the fulvic acid and dissolved organic matter fractions extracted from the same soil horizon using conventional techniques .
	manualset3
118179	1	404666	5	NULL	NULL	0	NULL	carboxyl-terminal CAP domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the carboxyl-terminal CAP domain is more similar to Na-ASP-2 than to the amino-terminal CAP domain .
	manualset3
118180	2	404666	5	NULL	NULL	0	NULL	Na-ASP-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the carboxyl-terminal CAP domain is more similar to Na-ASP-2 than to the amino-terminal CAP domain .
	manualset3
118181	3	404666	5	NULL	NULL	0	NULL	amino-terminal CAP domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the carboxyl-terminal CAP domain is more similar to Na-ASP-2 than to the amino-terminal CAP domain .
	manualset3
118182	1	404667	5	NULL	NULL	0	NULL	finite-element analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A finite-element analysis is used to explore the impact of elastic material properties , boundary conditions , and geometry , including coiling , on the spatial characteristics of the compliance of the unloaded basilar membrane ( BM ) .
	manualset3
118183	2	404667	5	NULL	NULL	0	NULL	impact 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A finite-element analysis is used to explore the impact of elastic material properties , boundary conditions , and geometry , including coiling , on the spatial characteristics of the compliance of the unloaded basilar membrane ( BM ) .
	manualset3
118184	3	404667	5	NULL	NULL	0	NULL	elastic material properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A finite-element analysis is used to explore the impact of elastic material properties , boundary conditions , and geometry , including coiling , on the spatial characteristics of the compliance of the unloaded basilar membrane ( BM ) .
	manualset3
118185	4	404667	5	NULL	NULL	0	NULL	boundary conditions	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A finite-element analysis is used to explore the impact of elastic material properties , boundary conditions , and geometry , including coiling , on the spatial characteristics of the compliance of the unloaded basilar membrane ( BM ) .
	manualset3
118186	5	404667	5	NULL	NULL	0	NULL	geometry 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A finite-element analysis is used to explore the impact of elastic material properties , boundary conditions , and geometry , including coiling , on the spatial characteristics of the compliance of the unloaded basilar membrane ( BM ) .
	manualset3
118187	6	404667	5	NULL	NULL	0	NULL	spatial characteristics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A finite-element analysis is used to explore the impact of elastic material properties , boundary conditions , and geometry , including coiling , on the spatial characteristics of the compliance of the unloaded basilar membrane ( BM ) .
	manualset3
118188	7	404667	5	NULL	NULL	0	NULL	compliance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A finite-element analysis is used to explore the impact of elastic material properties , boundary conditions , and geometry , including coiling , on the spatial characteristics of the compliance of the unloaded basilar membrane ( BM ) .
	manualset3
118189	8	404667	5	NULL	NULL	0	NULL	unloaded basilar membrane ( BM )	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A finite-element analysis is used to explore the impact of elastic material properties , boundary conditions , and geometry , including coiling , on the spatial characteristics of the compliance of the unloaded basilar membrane ( BM ) .
	manualset3
118190	1	404668	5	NULL	NULL	0	NULL	adiponectin concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the increase of adiponectin concentrations during ISIS 113715 treatment was correlated with the lowering of insulin responses during IVGTT ( r = -0.47 , P = 0.042 ) .
	manualset3
118191	2	404668	5	NULL	NULL	0	NULL	ISIS 113715 treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the increase of adiponectin concentrations during ISIS 113715 treatment was correlated with the lowering of insulin responses during IVGTT ( r = -0.47 , P = 0.042 ) .
	manualset3
118192	3	404668	5	NULL	NULL	0	NULL	insulin responses	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the increase of adiponectin concentrations during ISIS 113715 treatment was correlated with the lowering of insulin responses during IVGTT ( r = -0.47 , P = 0.042 ) .
	manualset3
118193	4	404668	5	NULL	NULL	0	NULL	IVGTT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the increase of adiponectin concentrations during ISIS 113715 treatment was correlated with the lowering of insulin responses during IVGTT ( r = -0.47 , P = 0.042 ) .
	manualset3
118194	5	404668	5	NULL	NULL	0	NULL	r = -0.47	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the increase of adiponectin concentrations during ISIS 113715 treatment was correlated with the lowering of insulin responses during IVGTT ( r = -0.47 , P = 0.042 ) .
	manualset3
118195	6	404668	5	NULL	NULL	0	NULL	P = 0.042	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the increase of adiponectin concentrations during ISIS 113715 treatment was correlated with the lowering of insulin responses during IVGTT ( r = -0.47 , P = 0.042 ) .
	manualset3
118220	1	404669	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the results presented here show that sizeable nearest-neighbor effects are seen only for residues preceding proline , where Pro introduces an overestimation , on average , of 1.73 ppm in the computed ( 13 ) C ( alpha ) chemical shifts .
	manualset3
118221	2	404669	5	NULL	NULL	0	NULL	nearest-neighbor effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the results presented here show that sizeable nearest-neighbor effects are seen only for residues preceding proline , where Pro introduces an overestimation , on average , of 1.73 ppm in the computed ( 13 ) C ( alpha ) chemical shifts .
	manualset3
118222	3	404669	5	NULL	NULL	NULL	NULL	residues preceding proline 	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Overall , the results presented here show that sizeable nearest-neighbor effects are seen only for residues preceding proline , where Pro introduces an overestimation , on average , of 1.73 ppm in the computed ( 13 ) C ( alpha ) chemical shifts .
	manualset3
118223	4	404669	5	NULL	NULL	0	NULL	Pro 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the results presented here show that sizeable nearest-neighbor effects are seen only for residues preceding proline , where Pro introduces an overestimation , on average , of 1.73 ppm in the computed ( 13 ) C ( alpha ) chemical shifts .
	manualset3
118224	5	404669	5	NULL	NULL	0	NULL	overestimation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the results presented here show that sizeable nearest-neighbor effects are seen only for residues preceding proline , where Pro introduces an overestimation , on average , of 1.73 ppm in the computed ( 13 ) C ( alpha ) chemical shifts .
	manualset3
118225	6	404669	5	NULL	NULL	0	NULL	average 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the results presented here show that sizeable nearest-neighbor effects are seen only for residues preceding proline , where Pro introduces an overestimation , on average , of 1.73 ppm in the computed ( 13 ) C ( alpha ) chemical shifts .
	manualset3
118226	7	404669	5	NULL	NULL	0	NULL	 1.73 ppm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the results presented here show that sizeable nearest-neighbor effects are seen only for residues preceding proline , where Pro introduces an overestimation , on average , of 1.73 ppm in the computed ( 13 ) C ( alpha ) chemical shifts .
	manualset3
118227	8	404669	5	NULL	NULL	0	NULL	 ( 13 ) C ( alpha ) chemical shifts	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the results presented here show that sizeable nearest-neighbor effects are seen only for residues preceding proline , where Pro introduces an overestimation , on average , of 1.73 ppm in the computed ( 13 ) C ( alpha ) chemical shifts .
	manualset3
118228	1	404670	5	NULL	NULL	0	NULL	inverse relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , there seems to be an inverse relationship between body mass index and testosterone levels , as is also demonstrated in our cross-sectional study .
	manualset3
118229	2	404670	5	NULL	NULL	0	NULL	body mass index	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , there seems to be an inverse relationship between body mass index and testosterone levels , as is also demonstrated in our cross-sectional study .
	manualset3
118230	3	404670	5	NULL	NULL	0	NULL	testosterone levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , there seems to be an inverse relationship between body mass index and testosterone levels , as is also demonstrated in our cross-sectional study .
	manualset3
118231	4	404670	5	NULL	NULL	0	NULL	cross-sectional study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , there seems to be an inverse relationship between body mass index and testosterone levels , as is also demonstrated in our cross-sectional study .
	manualset3
118232	1	404671	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , these data implicate Twist1 as a critical regulator of valve development and suggest that Twist1 influences ECM production and cell proliferation during disease .
	manualset3
118233	2	404671	5	NULL	NULL	0	NULL	Twist1 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , these data implicate Twist1 as a critical regulator of valve development and suggest that Twist1 influences ECM production and cell proliferation during disease .
	manualset3
118234	3	404671	5	NULL	NULL	0	NULL	critical regulator	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , these data implicate Twist1 as a critical regulator of valve development and suggest that Twist1 influences ECM production and cell proliferation during disease .
	manualset3
118235	4	404671	5	NULL	NULL	0	NULL	valve development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , these data implicate Twist1 as a critical regulator of valve development and suggest that Twist1 influences ECM production and cell proliferation during disease .
	manualset3
118236	5	404671	5	NULL	NULL	0	NULL	Twist1 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , these data implicate Twist1 as a critical regulator of valve development and suggest that Twist1 influences ECM production and cell proliferation during disease .
	manualset3
118237	6	404671	5	NULL	NULL	0	NULL	ECM production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , these data implicate Twist1 as a critical regulator of valve development and suggest that Twist1 influences ECM production and cell proliferation during disease .
	manualset3
118238	7	404671	5	NULL	NULL	0	NULL	cell proliferation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , these data implicate Twist1 as a critical regulator of valve development and suggest that Twist1 influences ECM production and cell proliferation during disease .
	manualset3
118239	8	404671	5	NULL	NULL	0	NULL	disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , these data implicate Twist1 as a critical regulator of valve development and suggest that Twist1 influences ECM production and cell proliferation during disease .
	manualset3
118240	1	404672	5	NULL	NULL	0	NULL	findings 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , these findings confirm that coevolutionary - methods can be confidently used in predicting PPI , either independently or as drivers of coimmunoprecipitation experiments .
	manualset3
118241	2	404672	5	NULL	NULL	0	NULL	coevolutionary - methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , these findings confirm that coevolutionary - methods can be confidently used in predicting PPI , either independently or as drivers of coimmunoprecipitation experiments .
	manualset3
118242	3	404672	5	NULL	NULL	0	NULL	PPI 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , these findings confirm that coevolutionary - methods can be confidently used in predicting PPI , either independently or as drivers of coimmunoprecipitation experiments .
	manualset3
118243	4	404672	5	NULL	NULL	0	NULL	coimmunoprecipitation experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , these findings confirm that coevolutionary - methods can be confidently used in predicting PPI , either independently or as drivers of coimmunoprecipitation experiments .
	manualset3
118244	1	404673	5	NULL	NULL	0	NULL	information 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , this information indicates that aberrant glutamate signaling may contribute to the development of some white matter pathologies .
	manualset3
118245	2	404673	5	NULL	NULL	0	NULL	glutamate signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , this information indicates that aberrant glutamate signaling may contribute to the development of some white matter pathologies .
	manualset3
118246	3	404673	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , this information indicates that aberrant glutamate signaling may contribute to the development of some white matter pathologies .
	manualset3
118247	4	404673	5	NULL	NULL	0	NULL	white matter pathologies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , this information indicates that aberrant glutamate signaling may contribute to the development of some white matter pathologies .
	manualset3
118248	1	404674	5	NULL	NULL	0	NULL	pattern 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , this pattern is very similar to the pattern of breast cancer in Nigerian women .
	manualset3
118249	2	404674	5	NULL	NULL	0	NULL	pattern 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , this pattern is very similar to the pattern of breast cancer in Nigerian women .
	manualset3
118250	3	404674	5	NULL	NULL	0	NULL	breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , this pattern is very similar to the pattern of breast cancer in Nigerian women .
	manualset3
118251	4	404674	5	NULL	NULL	0	NULL	Nigerian women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , this pattern is very similar to the pattern of breast cancer in Nigerian women .
	manualset3
118252	1	404675	5	NULL	NULL	0	NULL	total vegetable intake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , total vegetable intake was not associated with pancreatic cancer risk , nor was intake of vegetable subgroups .
	manualset3
118253	2	404675	5	NULL	NULL	0	NULL	pancreatic cancer risk	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , total vegetable intake was not associated with pancreatic cancer risk , nor was intake of vegetable subgroups .
	manualset3
118254	3	404675	5	NULL	NULL	0	NULL	intake 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , total vegetable intake was not associated with pancreatic cancer risk , nor was intake of vegetable subgroups .
	manualset3
118255	4	404675	5	NULL	NULL	0	NULL	vegetable subgroups	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , total vegetable intake was not associated with pancreatic cancer risk , nor was intake of vegetable subgroups .
	manualset3
118256	1	404676	5	NULL	NULL	0	NULL	supplemented 3-month-old mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall the supplemented 3-month-old mice exhibited both higher lymphoproliferative responses and production of cytokines compared with the supplemented 6-month-old mice .
	manualset3
118257	2	404676	5	NULL	NULL	0	NULL	higher lymphoproliferative responses 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall the supplemented 3-month-old mice exhibited both higher lymphoproliferative responses and production of cytokines compared with the supplemented 6-month-old mice .
	manualset3
118258	3	404676	5	NULL	NULL	0	NULL	production 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall the supplemented 3-month-old mice exhibited both higher lymphoproliferative responses and production of cytokines compared with the supplemented 6-month-old mice .
	manualset3
118259	4	404676	5	NULL	NULL	0	NULL	cytokines 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall the supplemented 3-month-old mice exhibited both higher lymphoproliferative responses and production of cytokines compared with the supplemented 6-month-old mice .
	manualset3
118260	5	404676	5	NULL	NULL	0	NULL	supplemented 6-month-old mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall the supplemented 3-month-old mice exhibited both higher lymphoproliferative responses and production of cytokines compared with the supplemented 6-month-old mice .
	manualset3
118261	1	404677	5	NULL	NULL	0	NULL	Overexpressed gelsolin protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpressed gelsolin protein was cleaved during apoptosis , as seen previously in this and other cell types .
	manualset3
118262	2	404677	5	NULL	NULL	0	NULL	apoptosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpressed gelsolin protein was cleaved during apoptosis , as seen previously in this and other cell types .
	manualset3
118263	3	404677	5	NULL	NULL	0	NULL	cell types	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpressed gelsolin protein was cleaved during apoptosis , as seen previously in this and other cell types .
	manualset3
118264	1	404678	5	NULL	NULL	NULL	NULL	Overexpression 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Overexpression , purification , crystallization and preliminary crystallographic studies of a hyperthermophilic adenylosuccinate synthetase from Pyrococcus horikoshii OT3 .
	manualset3
118265	2	404678	5	NULL	NULL	0	NULL	purification 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression , purification , crystallization and preliminary crystallographic studies of a hyperthermophilic adenylosuccinate synthetase from Pyrococcus horikoshii OT3 .
	manualset3
118266	3	404678	5	NULL	NULL	0	NULL	crystallization 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression , purification , crystallization and preliminary crystallographic studies of a hyperthermophilic adenylosuccinate synthetase from Pyrococcus horikoshii OT3 .
	manualset3
118267	4	404678	5	NULL	NULL	0	NULL	preliminary crystallographic studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression , purification , crystallization and preliminary crystallographic studies of a hyperthermophilic adenylosuccinate synthetase from Pyrococcus horikoshii OT3 .
	manualset3
118268	5	404678	5	NULL	NULL	NULL	NULL	hyperthermophilic adenylosuccinate synthetase	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Overexpression , purification , crystallization and preliminary crystallographic studies of a hyperthermophilic adenylosuccinate synthetase from Pyrococcus horikoshii OT3 .
	manualset3
118269	6	404678	5	NULL	NULL	0	NULL	Pyrococcus horikoshii OT3	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression , purification , crystallization and preliminary crystallographic studies of a hyperthermophilic adenylosuccinate synthetase from Pyrococcus horikoshii OT3 .
	manualset3
118270	1	404679	5	NULL	NULL	NULL	NULL	Overexpression 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Overexpression of BMP3 in chick wing bud at the onset of chondrogenesis , using replication competent retrovirus , reduces BMP signaling leading to increased cell proliferation and delayed cell differentiation , resulting in expanded skeletal elements and joint fusions .
	manualset3
118271	2	404679	5	NULL	NULL	NULL	NULL	BMP3 	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Overexpression of BMP3 in chick wing bud at the onset of chondrogenesis , using replication competent retrovirus , reduces BMP signaling leading to increased cell proliferation and delayed cell differentiation , resulting in expanded skeletal elements and joint fusions .
	manualset3
118272	3	404679	5	NULL	NULL	0	NULL	chick wing bud	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of BMP3 in chick wing bud at the onset of chondrogenesis , using replication competent retrovirus , reduces BMP signaling leading to increased cell proliferation and delayed cell differentiation , resulting in expanded skeletal elements and joint fusions .
	manualset3
118273	4	404679	5	NULL	NULL	0	NULL	onset 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of BMP3 in chick wing bud at the onset of chondrogenesis , using replication competent retrovirus , reduces BMP signaling leading to increased cell proliferation and delayed cell differentiation , resulting in expanded skeletal elements and joint fusions .
	manualset3
118274	5	404679	5	NULL	NULL	0	NULL	chondrogenesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of BMP3 in chick wing bud at the onset of chondrogenesis , using replication competent retrovirus , reduces BMP signaling leading to increased cell proliferation and delayed cell differentiation , resulting in expanded skeletal elements and joint fusions .
	manualset3
118275	6	404679	5	NULL	NULL	0	NULL	BMP signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of BMP3 in chick wing bud at the onset of chondrogenesis , using replication competent retrovirus , reduces BMP signaling leading to increased cell proliferation and delayed cell differentiation , resulting in expanded skeletal elements and joint fusions .
	manualset3
118276	7	404679	5	NULL	NULL	NULL	NULL	increased cell proliferation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Overexpression of BMP3 in chick wing bud at the onset of chondrogenesis , using replication competent retrovirus , reduces BMP signaling leading to increased cell proliferation and delayed cell differentiation , resulting in expanded skeletal elements and joint fusions .
	manualset3
118277	8	404679	5	NULL	NULL	NULL	NULL	delayed cell differentiation 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Overexpression of BMP3 in chick wing bud at the onset of chondrogenesis , using replication competent retrovirus , reduces BMP signaling leading to increased cell proliferation and delayed cell differentiation , resulting in expanded skeletal elements and joint fusions .
	manualset3
118278	9	404679	5	NULL	NULL	0	NULL	expanded skeletal elements	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of BMP3 in chick wing bud at the onset of chondrogenesis , using replication competent retrovirus , reduces BMP signaling leading to increased cell proliferation and delayed cell differentiation , resulting in expanded skeletal elements and joint fusions .
	manualset3
118279	10	404679	5	NULL	NULL	0	NULL	joint fusions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of BMP3 in chick wing bud at the onset of chondrogenesis , using replication competent retrovirus , reduces BMP signaling leading to increased cell proliferation and delayed cell differentiation , resulting in expanded skeletal elements and joint fusions .
	manualset3
121234	11	404679	5	NULL	NULL	0	NULL	replication competent retrovirus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of BMP3 in chick wing bud at the onset of chondrogenesis , using replication competent retrovirus , reduces BMP signaling leading to increased cell proliferation and delayed cell differentiation , resulting in expanded skeletal elements and joint fusions .
	manualset3
118281	1	404680	5	NULL	NULL	NULL	NULL	Overexpression 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Overexpression of FGFR3 , Stat1 , Stat5 and p21Cip1 correlates with phenotypic severity and defective chondrocyte differentiation in FGFR3-related chondrodysplasias .
	manualset3
118282	2	404680	5	NULL	NULL	NULL	NULL	FGFR3 	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Overexpression of FGFR3 , Stat1 , Stat5 and p21Cip1 correlates with phenotypic severity and defective chondrocyte differentiation in FGFR3-related chondrodysplasias .
	manualset3
118283	3	404680	5	NULL	NULL	NULL	NULL	Stat1 	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Overexpression of FGFR3 , Stat1 , Stat5 and p21Cip1 correlates with phenotypic severity and defective chondrocyte differentiation in FGFR3-related chondrodysplasias .
	manualset3
118284	4	404680	5	NULL	NULL	0	NULL	Stat5 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of FGFR3 , Stat1 , Stat5 and p21Cip1 correlates with phenotypic severity and defective chondrocyte differentiation in FGFR3-related chondrodysplasias .
	manualset3
118285	5	404680	5	NULL	NULL	0	NULL	 p21Cip1	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of FGFR3 , Stat1 , Stat5 and p21Cip1 correlates with phenotypic severity and defective chondrocyte differentiation in FGFR3-related chondrodysplasias .
	manualset3
118286	6	404680	5	NULL	NULL	NULL	NULL	phenotypic severity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Overexpression of FGFR3 , Stat1 , Stat5 and p21Cip1 correlates with phenotypic severity and defective chondrocyte differentiation in FGFR3-related chondrodysplasias .
	manualset3
118287	7	404680	5	NULL	NULL	0	NULL	defective chondrocyte differentiation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of FGFR3 , Stat1 , Stat5 and p21Cip1 correlates with phenotypic severity and defective chondrocyte differentiation in FGFR3-related chondrodysplasias .
	manualset3
118288	8	404680	5	NULL	NULL	0	NULL	FGFR3-related chondrodysplasias	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of FGFR3 , Stat1 , Stat5 and p21Cip1 correlates with phenotypic severity and defective chondrocyte differentiation in FGFR3-related chondrodysplasias .
	manualset3
118289	1	404681	5	NULL	NULL	NULL	NULL	Overexpression 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Overexpression of FKBP38 blocks apoptosis , whereas functional inhibition of this protein by a dominant-negative mutant or by RNA interference promotes apoptosis .
	manualset3
118290	2	404681	5	NULL	NULL	0	NULL	FKBP38 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of FKBP38 blocks apoptosis , whereas functional inhibition of this protein by a dominant-negative mutant or by RNA interference promotes apoptosis .
	manualset3
118291	3	404681	5	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of FKBP38 blocks apoptosis , whereas functional inhibition of this protein by a dominant-negative mutant or by RNA interference promotes apoptosis .
	manualset3
118292	4	404681	5	NULL	NULL	NULL	NULL	functional inhibition	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Overexpression of FKBP38 blocks apoptosis , whereas functional inhibition of this protein by a dominant-negative mutant or by RNA interference promotes apoptosis .
	manualset3
118293	5	404681	5	NULL	NULL	0	NULL	protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of FKBP38 blocks apoptosis , whereas functional inhibition of this protein by a dominant-negative mutant or by RNA interference promotes apoptosis .
	manualset3
118294	6	404681	5	NULL	NULL	0	NULL	dominant-negative mutant	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of FKBP38 blocks apoptosis , whereas functional inhibition of this protein by a dominant-negative mutant or by RNA interference promotes apoptosis .
	manualset3
118295	7	404681	5	NULL	NULL	0	NULL	RNA interference	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of FKBP38 blocks apoptosis , whereas functional inhibition of this protein by a dominant-negative mutant or by RNA interference promotes apoptosis .
	manualset3
118296	8	404681	5	NULL	NULL	0	NULL	apoptosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of FKBP38 blocks apoptosis , whereas functional inhibition of this protein by a dominant-negative mutant or by RNA interference promotes apoptosis .
	manualset3
118297	1	404682	5	NULL	NULL	NULL	NULL	Overexpression 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Overexpression of Fer increases the association of tyrosine-phosphorylated IRS-1 with P85 phosphatidylinositol kinase via SH2 domain of Fer in transfected cells .
	manualset3
118298	2	404682	5	NULL	NULL	NULL	NULL	Fer 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Overexpression of Fer increases the association of tyrosine-phosphorylated IRS-1 with P85 phosphatidylinositol kinase via SH2 domain of Fer in transfected cells .
	manualset3
118302	3	404682	5	NULL	NULL	0	NULL	association 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of Fer increases the association of tyrosine-phosphorylated IRS-1 with P85 phosphatidylinositol kinase via SH2 domain of Fer in transfected cells .
	manualset3
118304	4	404682	5	NULL	NULL	0	NULL	tyrosine-phosphorylated IRS-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of Fer increases the association of tyrosine-phosphorylated IRS-1 with P85 phosphatidylinositol kinase via SH2 domain of Fer in transfected cells .
	manualset3
118305	5	404682	5	NULL	NULL	0	NULL	P85 phosphatidylinositol kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of Fer increases the association of tyrosine-phosphorylated IRS-1 with P85 phosphatidylinositol kinase via SH2 domain of Fer in transfected cells .
	manualset3
118306	6	404682	5	NULL	NULL	0	NULL	SH2 domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of Fer increases the association of tyrosine-phosphorylated IRS-1 with P85 phosphatidylinositol kinase via SH2 domain of Fer in transfected cells .
	manualset3
118307	7	404682	5	NULL	NULL	0	NULL	Fer	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of Fer increases the association of tyrosine-phosphorylated IRS-1 with P85 phosphatidylinositol kinase via SH2 domain of Fer in transfected cells .
	manualset3
118308	8	404682	5	NULL	NULL	0	NULL	transfected cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of Fer increases the association of tyrosine-phosphorylated IRS-1 with P85 phosphatidylinositol kinase via SH2 domain of Fer in transfected cells .
	manualset3
118309	1	404683	5	NULL	NULL	NULL	NULL	Overexpression 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Overexpression of MiD49/51 seems to sequester Drp1 from functioning at mitochondria and cause fused tubules to associate with actin .
	manualset3
118310	2	404683	5	NULL	NULL	0	NULL	MiD49/51	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of MiD49/51 seems to sequester Drp1 from functioning at mitochondria and cause fused tubules to associate with actin .
	manualset3
118311	3	404683	5	NULL	NULL	0	NULL	Drp1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of MiD49/51 seems to sequester Drp1 from functioning at mitochondria and cause fused tubules to associate with actin .
	manualset3
118312	4	404683	5	NULL	NULL	0	NULL	mitochondria 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of MiD49/51 seems to sequester Drp1 from functioning at mitochondria and cause fused tubules to associate with actin .
	manualset3
118313	5	404683	5	NULL	NULL	NULL	NULL	fused tubules	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Overexpression of MiD49/51 seems to sequester Drp1 from functioning at mitochondria and cause fused tubules to associate with actin .
	manualset3
118314	6	404683	5	NULL	NULL	NULL	NULL	actin 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Overexpression of MiD49/51 seems to sequester Drp1 from functioning at mitochondria and cause fused tubules to associate with actin .
	manualset3
118315	1	404684	5	NULL	NULL	0	NULL	Overexpression 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of SRK1 ( SSD1 ) , URE2 , DAL80 , MEP1 , or MEP3 suppressed only the growth defect of the Deltamep1/Deltamep1 Deltamep2/Deltamep2 mutant strain .
	manualset3
118325	2	404684	5	NULL	NULL	0	NULL	SRK1 ( SSD1 )	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of SRK1 ( SSD1 ) , URE2 , DAL80 , MEP1 , or MEP3 suppressed only the growth defect of the Deltamep1/Deltamep1 Deltamep2/Deltamep2 mutant strain .
	manualset3
118326	3	404684	5	NULL	NULL	0	NULL	URE2 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of SRK1 ( SSD1 ) , URE2 , DAL80 , MEP1 , or MEP3 suppressed only the growth defect of the Deltamep1/Deltamep1 Deltamep2/Deltamep2 mutant strain .
	manualset3
118327	4	404684	5	NULL	NULL	0	NULL	DAL80 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of SRK1 ( SSD1 ) , URE2 , DAL80 , MEP1 , or MEP3 suppressed only the growth defect of the Deltamep1/Deltamep1 Deltamep2/Deltamep2 mutant strain .
	manualset3
118328	5	404684	5	NULL	NULL	0	NULL	MEP1 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of SRK1 ( SSD1 ) , URE2 , DAL80 , MEP1 , or MEP3 suppressed only the growth defect of the Deltamep1/Deltamep1 Deltamep2/Deltamep2 mutant strain .
	manualset3
118329	6	404684	5	NULL	NULL	0	NULL	MEP3 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of SRK1 ( SSD1 ) , URE2 , DAL80 , MEP1 , or MEP3 suppressed only the growth defect of the Deltamep1/Deltamep1 Deltamep2/Deltamep2 mutant strain .
	manualset3
118330	7	404684	5	NULL	NULL	0	NULL	growth defect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of SRK1 ( SSD1 ) , URE2 , DAL80 , MEP1 , or MEP3 suppressed only the growth defect of the Deltamep1/Deltamep1 Deltamep2/Deltamep2 mutant strain .
	manualset3
118331	8	404684	5	NULL	NULL	0	NULL	Deltamep1/Deltamep1 Deltamep2/Deltamep2 mutant strain	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of SRK1 ( SSD1 ) , URE2 , DAL80 , MEP1 , or MEP3 suppressed only the growth defect of the Deltamep1/Deltamep1 Deltamep2/Deltamep2 mutant strain .
	manualset3
118332	1	404685	5	NULL	NULL	0	NULL	Overexpression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of Wnt3 in the lateral tectum repelled the termination zones of dorsal RGC axons in vivo .
	manualset3
118333	2	404685	5	NULL	NULL	0	NULL	Wnt3 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of Wnt3 in the lateral tectum repelled the termination zones of dorsal RGC axons in vivo .
	manualset3
118334	3	404685	5	NULL	NULL	0	NULL	lateral tectum	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of Wnt3 in the lateral tectum repelled the termination zones of dorsal RGC axons in vivo .
	manualset3
118335	4	404685	5	NULL	NULL	NULL	NULL	termination zones	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Overexpression of Wnt3 in the lateral tectum repelled the termination zones of dorsal RGC axons in vivo .
	manualset3
118336	5	404685	5	NULL	NULL	0	NULL	dorsal RGC axons 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of Wnt3 in the lateral tectum repelled the termination zones of dorsal RGC axons in vivo .
	manualset3
118338	1	404686	5	NULL	NULL	0	NULL	Overexpression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of gelsolin in human cervical carcinoma and its clinicopathological significance .
	manualset3
118341	2	404686	5	NULL	NULL	NULL	NULL	gelsolin 	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Overexpression of gelsolin in human cervical carcinoma and its clinicopathological significance .
	manualset3
118342	3	404686	5	NULL	NULL	0	NULL	human cervical carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of gelsolin in human cervical carcinoma and its clinicopathological significance .
	manualset3
118344	4	404686	5	NULL	NULL	0	NULL	clinicopathological significance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of gelsolin in human cervical carcinoma and its clinicopathological significance .
	manualset3
118345	1	404687	5	NULL	NULL	0	NULL	Overexpression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of the ABC transporter AvtAB increases avermectin production in Streptomyces avermitilis .
	manualset3
118346	2	404687	5	NULL	NULL	0	NULL	ABC transporter AvtAB 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of the ABC transporter AvtAB increases avermectin production in Streptomyces avermitilis .
	manualset3
118347	3	404687	5	NULL	NULL	0	NULL	avermectin production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of the ABC transporter AvtAB increases avermectin production in Streptomyces avermitilis .
	manualset3
118348	4	404687	5	NULL	NULL	0	NULL	Streptomyces avermitilis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of the ABC transporter AvtAB increases avermectin production in Streptomyces avermitilis .
	manualset3
118349	1	404688	5	NULL	NULL	NULL	NULL	adolescent dams	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Overnourishing the adolescent dams to promote rapid maternal growth throughout pregnancy results in a major restriction in placental mass and leads to a significant decrease in birth weight relative to moderately-fed adolescents of equivalent gynaecological age .
	manualset3
118350	2	404688	5	NULL	NULL	0	NULL	rapid maternal growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overnourishing the adolescent dams to promote rapid maternal growth throughout pregnancy results in a major restriction in placental mass and leads to a significant decrease in birth weight relative to moderately-fed adolescents of equivalent gynaecological age .
	manualset3
118351	3	404688	5	NULL	NULL	0	NULL	pregnancy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Overnourishing the adolescent dams to promote rapid maternal growth throughout pregnancy results in a major restriction in placental mass and leads to a significant decrease in birth weight relative to moderately-fed adolescents of equivalent gynaecological age .
	manualset3
118352	4	404688	5	NULL	NULL	0	NULL	major restriction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Overnourishing the adolescent dams to promote rapid maternal growth throughout pregnancy results in a major restriction in placental mass and leads to a significant decrease in birth weight relative to moderately-fed adolescents of equivalent gynaecological age .
	manualset3
118353	5	404688	5	NULL	NULL	0	NULL	placental mass 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Overnourishing the adolescent dams to promote rapid maternal growth throughout pregnancy results in a major restriction in placental mass and leads to a significant decrease in birth weight relative to moderately-fed adolescents of equivalent gynaecological age .
	manualset3
118354	6	404688	5	NULL	NULL	0	NULL	birth weight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overnourishing the adolescent dams to promote rapid maternal growth throughout pregnancy results in a major restriction in placental mass and leads to a significant decrease in birth weight relative to moderately-fed adolescents of equivalent gynaecological age .
	manualset3
118355	7	404688	5	NULL	NULL	0	NULL	moderately-fed adolescents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Overnourishing the adolescent dams to promote rapid maternal growth throughout pregnancy results in a major restriction in placental mass and leads to a significant decrease in birth weight relative to moderately-fed adolescents of equivalent gynaecological age .
	manualset3
118356	8	404688	5	NULL	NULL	0	NULL	equivalent gynaecological age	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Overnourishing the adolescent dams to promote rapid maternal growth throughout pregnancy results in a major restriction in placental mass and leads to a significant decrease in birth weight relative to moderately-fed adolescents of equivalent gynaecological age .
	manualset3
121235	9	404688	5	NULL	NULL	0	NULL	decrease 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Overnourishing the adolescent dams to promote rapid maternal growth throughout pregnancy results in a major restriction in placental mass and leads to a significant decrease in birth weight relative to moderately-fed adolescents of equivalent gynaecological age .
	manualset3
118357	1	404689	5	NULL	NULL	0	NULL	Overview 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Overview of the treatment of acne vulgaris with topical retinoids .
	manualset3
118358	2	404689	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Overview of the treatment of acne vulgaris with topical retinoids .
	manualset3
118359	3	404689	5	NULL	NULL	0	NULL	acne vulgaris	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Overview of the treatment of acne vulgaris with topical retinoids .
	manualset3
118360	4	404689	5	NULL	NULL	0	NULL	topical retinoids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Overview of the treatment of acne vulgaris with topical retinoids .
	manualset3
118361	1	404690	5	NULL	NULL	0	NULL	Overweight 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Overweight and obesity among children with developmental disabilities .
	manualset3
118362	2	404690	5	NULL	NULL	0	NULL	obesity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Overweight and obesity among children with developmental disabilities .
	manualset3
118363	3	404690	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Overweight and obesity among children with developmental disabilities .
	manualset3
118364	4	404690	5	NULL	NULL	0	NULL	developmental disabilities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Overweight and obesity among children with developmental disabilities .
	manualset3
118365	1	404691	5	NULL	NULL	0	NULL	malpractice suits	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Owing to a massive increase in malpractice suits directed against dentists and an escalation in the amount of settlements and court ordered awards , professional liability premiums are increasing at an alarming rate .
	manualset3
118366	2	404691	5	NULL	NULL	0	NULL	dentists 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Owing to a massive increase in malpractice suits directed against dentists and an escalation in the amount of settlements and court ordered awards , professional liability premiums are increasing at an alarming rate .
	manualset3
118367	3	404691	5	NULL	NULL	0	NULL	escalation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Owing to a massive increase in malpractice suits directed against dentists and an escalation in the amount of settlements and court ordered awards , professional liability premiums are increasing at an alarming rate .
	manualset3
118368	4	404691	5	NULL	NULL	0	NULL	amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Owing to a massive increase in malpractice suits directed against dentists and an escalation in the amount of settlements and court ordered awards , professional liability premiums are increasing at an alarming rate .
	manualset3
118369	5	404691	5	NULL	NULL	0	NULL	settlements 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Owing to a massive increase in malpractice suits directed against dentists and an escalation in the amount of settlements and court ordered awards , professional liability premiums are increasing at an alarming rate .
	manualset3
118370	6	404691	5	NULL	NULL	0	NULL	court ordered awards	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Owing to a massive increase in malpractice suits directed against dentists and an escalation in the amount of settlements and court ordered awards , professional liability premiums are increasing at an alarming rate .
	manualset3
118371	7	404691	5	NULL	NULL	0	NULL	professional liability premiums	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Owing to a massive increase in malpractice suits directed against dentists and an escalation in the amount of settlements and court ordered awards , professional liability premiums are increasing at an alarming rate .
	manualset3
118372	8	404691	5	NULL	NULL	0	NULL	alarming rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Owing to a massive increase in malpractice suits directed against dentists and an escalation in the amount of settlements and court ordered awards , professional liability premiums are increasing at an alarming rate .
	manualset3
121236	9	404691	5	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Owing to a massive increase in malpractice suits directed against dentists and an escalation in the amount of settlements and court ordered awards , professional liability premiums are increasing at an alarming rate .
	manualset3
118375	1	404692	5	NULL	NULL	NULL	NULL	pyridone end unit	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Owing to its pyridone end unit , BIQ 3 can display different resonance structures in different solvents ( aprotic and protic ) or Lewis acids to give different colors .
	manualset3
118376	2	404692	5	NULL	NULL	0	NULL	resonance structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Owing to its pyridone end unit , BIQ 3 can display different resonance structures in different solvents ( aprotic and protic ) or Lewis acids to give different colors .
	manualset3
118377	3	404692	5	NULL	NULL	0	NULL	different solvents ( aprotic and protic ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Owing to its pyridone end unit , BIQ 3 can display different resonance structures in different solvents ( aprotic and protic ) or Lewis acids to give different colors .
	manualset3
118378	4	404692	5	NULL	NULL	0	NULL	Lewis acids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Owing to its pyridone end unit , BIQ 3 can display different resonance structures in different solvents ( aprotic and protic ) or Lewis acids to give different colors .
	manualset3
118379	5	404692	5	NULL	NULL	0	NULL	different colors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Owing to its pyridone end unit , BIQ 3 can display different resonance structures in different solvents ( aprotic and protic ) or Lewis acids to give different colors .
	manualset3
121237	6	404692	5	NULL	NULL	0	NULL	BIQ 3	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Owing to its pyridone end unit , BIQ 3 can display different resonance structures in different solvents ( aprotic and protic ) or Lewis acids to give different colors .
	manualset3
118380	1	404693	5	NULL	NULL	0	NULL	close proximity 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Owing to the close proximity of the donor and acceptor entities , strong pi-pi intramolecular interactions between the porphyrin and fullerene entities resulted in modulating the spectral and electrochemical properties of the dyads .
	manualset3
118381	2	404693	5	NULL	NULL	0	NULL	donor entities 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Owing to the close proximity of the donor and acceptor entities , strong pi-pi intramolecular interactions between the porphyrin and fullerene entities resulted in modulating the spectral and electrochemical properties of the dyads .
	manualset3
118382	3	404693	5	NULL	NULL	0	NULL	 acceptor entities 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Owing to the close proximity of the donor and acceptor entities , strong pi-pi intramolecular interactions between the porphyrin and fullerene entities resulted in modulating the spectral and electrochemical properties of the dyads .
	manualset3
118383	4	404693	5	NULL	NULL	0	NULL	pi-pi intramolecular interactions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Owing to the close proximity of the donor and acceptor entities , strong pi-pi intramolecular interactions between the porphyrin and fullerene entities resulted in modulating the spectral and electrochemical properties of the dyads .
	manualset3
118388	5	404693	5	NULL	NULL	0	NULL	porphyrin 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Owing to the close proximity of the donor and acceptor entities , strong pi-pi intramolecular interactions between the porphyrin and fullerene entities resulted in modulating the spectral and electrochemical properties of the dyads .
	manualset3
118393	6	404693	5	NULL	NULL	0	NULL	fullerene entities	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Owing to the close proximity of the donor and acceptor entities , strong pi-pi intramolecular interactions between the porphyrin and fullerene entities resulted in modulating the spectral and electrochemical properties of the dyads .
	manualset3
118396	7	404693	5	NULL	NULL	0	NULL	spectral properties 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Owing to the close proximity of the donor and acceptor entities , strong pi-pi intramolecular interactions between the porphyrin and fullerene entities resulted in modulating the spectral and electrochemical properties of the dyads .
	manualset3
118398	8	404693	5	NULL	NULL	0	NULL	electrochemical properties 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Owing to the close proximity of the donor and acceptor entities , strong pi-pi intramolecular interactions between the porphyrin and fullerene entities resulted in modulating the spectral and electrochemical properties of the dyads .
	manualset3
118401	9	404693	5	NULL	NULL	0	NULL	dyads 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Owing to the close proximity of the donor and acceptor entities , strong pi-pi intramolecular interactions between the porphyrin and fullerene entities resulted in modulating the spectral and electrochemical properties of the dyads .
	manualset3
118404	1	404694	5	NULL	NULL	0	NULL	five-step synthesis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A five-step synthesis of the natural product angelicoin A using a late stage highly regioselective palladium ( 0 ) - catalyzed decarboxylative prenyl migration and aromatization sequence as the key step is reported .
	manualset3
118405	2	404694	5	NULL	NULL	0	NULL	natural product angelicoin A 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A five-step synthesis of the natural product angelicoin A using a late stage highly regioselective palladium ( 0 ) - catalyzed decarboxylative prenyl migration and aromatization sequence as the key step is reported .
	manualset3
118407	3	404694	5	NULL	NULL	0	NULL	palladium ( 0 ) - catalyzed decarboxylative prenyl migration	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A five-step synthesis of the natural product angelicoin A using a late stage highly regioselective palladium ( 0 ) - catalyzed decarboxylative prenyl migration and aromatization sequence as the key step is reported .
	manualset3
118408	4	404694	5	NULL	NULL	0	NULL	aromatization sequence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A five-step synthesis of the natural product angelicoin A using a late stage highly regioselective palladium ( 0 ) - catalyzed decarboxylative prenyl migration and aromatization sequence as the key step is reported .
	manualset3
118409	5	404694	5	NULL	NULL	0	NULL	key step	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A five-step synthesis of the natural product angelicoin A using a late stage highly regioselective palladium ( 0 ) - catalyzed decarboxylative prenyl migration and aromatization sequence as the key step is reported .
	manualset3
118411	1	404695	5	NULL	NULL	0	NULL	Oxidant insults	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidant insults can lead to apoptotic and nonapoptotic cell death .
	manualset3
118412	2	404695	5	NULL	NULL	0	NULL	apoptotic cell death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidant insults can lead to apoptotic and nonapoptotic cell death .
	manualset3
118413	3	404695	5	NULL	NULL	0	NULL	nonapoptotic cell death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidant insults can lead to apoptotic and nonapoptotic cell death .
	manualset3
118416	1	404696	5	NULL	NULL	0	NULL	Oxidants 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidants , antioxidants , and the beneficial roles of exercise-induced production of reactive species .
	manualset3
118417	2	404696	5	NULL	NULL	0	NULL	antioxidants 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidants , antioxidants , and the beneficial roles of exercise-induced production of reactive species .
	manualset3
118419	3	404696	5	NULL	NULL	0	NULL	beneficial roles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidants , antioxidants , and the beneficial roles of exercise-induced production of reactive species .
	manualset3
118421	4	404696	5	NULL	NULL	0	NULL	exercise-induced production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidants , antioxidants , and the beneficial roles of exercise-induced production of reactive species .
	manualset3
118422	5	404696	5	NULL	NULL	0	NULL	reactive species	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidants , antioxidants , and the beneficial roles of exercise-induced production of reactive species .
	manualset3
118423	1	404697	5	NULL	NULL	0	NULL	Oxidation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidation of LDL was initiated by addition of CuSO4 and monitored for production of conjugated dienes , thiobarbituric acid reactive substances ( TBARS ) and lipid peroxides .
	manualset3
118424	2	404697	5	NULL	NULL	0	NULL	LDL 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidation of LDL was initiated by addition of CuSO4 and monitored for production of conjugated dienes , thiobarbituric acid reactive substances ( TBARS ) and lipid peroxides .
	manualset3
118426	3	404697	5	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidation of LDL was initiated by addition of CuSO4 and monitored for production of conjugated dienes , thiobarbituric acid reactive substances ( TBARS ) and lipid peroxides .
	manualset3
118427	4	404697	5	NULL	NULL	0	NULL	CuSO4 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidation of LDL was initiated by addition of CuSO4 and monitored for production of conjugated dienes , thiobarbituric acid reactive substances ( TBARS ) and lipid peroxides .
	manualset3
118431	5	404697	5	NULL	NULL	0	NULL	production 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidation of LDL was initiated by addition of CuSO4 and monitored for production of conjugated dienes , thiobarbituric acid reactive substances ( TBARS ) and lipid peroxides .
	manualset3
118437	6	404697	5	NULL	NULL	0	NULL	conjugated dienes	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidation of LDL was initiated by addition of CuSO4 and monitored for production of conjugated dienes , thiobarbituric acid reactive substances ( TBARS ) and lipid peroxides .
	manualset3
118440	7	404697	5	NULL	NULL	0	NULL	thiobarbituric acid reactive substances ( TBARS ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidation of LDL was initiated by addition of CuSO4 and monitored for production of conjugated dienes , thiobarbituric acid reactive substances ( TBARS ) and lipid peroxides .
	manualset3
118442	8	404697	5	NULL	NULL	0	NULL	lipid peroxides	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidation of LDL was initiated by addition of CuSO4 and monitored for production of conjugated dienes , thiobarbituric acid reactive substances ( TBARS ) and lipid peroxides .
	manualset3
118444	1	404698	5	NULL	NULL	0	NULL	Oxidative stress	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidative stress induces cell death and growth arrest .
	manualset3
118445	2	404698	5	NULL	NULL	0	NULL	cell death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidative stress induces cell death and growth arrest .
	manualset3
118447	3	404698	5	NULL	NULL	0	NULL	growth arrest	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidative stress induces cell death and growth arrest .
	manualset3
118450	1	404699	5	NULL	NULL	0	NULL	Oxidative stress	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidative stress possibly via the modification of cysteine residues activates multiple stress kinase pathways and transcription factors nuclear factor-kappaB and activator protein-1 , which differentially regulate the genes for proinflammatory cytokines as well as the protective antioxidant genes .
	manualset3
118451	2	404699	5	NULL	NULL	0	NULL	modification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidative stress possibly via the modification of cysteine residues activates multiple stress kinase pathways and transcription factors nuclear factor-kappaB and activator protein-1 , which differentially regulate the genes for proinflammatory cytokines as well as the protective antioxidant genes .
	manualset3
118452	3	404699	5	NULL	NULL	0	NULL	cysteine residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidative stress possibly via the modification of cysteine residues activates multiple stress kinase pathways and transcription factors nuclear factor-kappaB and activator protein-1 , which differentially regulate the genes for proinflammatory cytokines as well as the protective antioxidant genes .
	manualset3
118453	4	404699	5	NULL	NULL	0	NULL	multiple stress kinase pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidative stress possibly via the modification of cysteine residues activates multiple stress kinase pathways and transcription factors nuclear factor-kappaB and activator protein-1 , which differentially regulate the genes for proinflammatory cytokines as well as the protective antioxidant genes .
	manualset3
118454	5	404699	5	NULL	NULL	0	NULL	transcription factors nuclear factor-kappaB	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidative stress possibly via the modification of cysteine residues activates multiple stress kinase pathways and transcription factors nuclear factor-kappaB and activator protein-1 , which differentially regulate the genes for proinflammatory cytokines as well as the protective antioxidant genes .
	manualset3
118456	6	404699	5	NULL	NULL	0	NULL	activator protein-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidative stress possibly via the modification of cysteine residues activates multiple stress kinase pathways and transcription factors nuclear factor-kappaB and activator protein-1 , which differentially regulate the genes for proinflammatory cytokines as well as the protective antioxidant genes .
	manualset3
118457	7	404699	5	NULL	NULL	0	NULL	genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidative stress possibly via the modification of cysteine residues activates multiple stress kinase pathways and transcription factors nuclear factor-kappaB and activator protein-1 , which differentially regulate the genes for proinflammatory cytokines as well as the protective antioxidant genes .
	manualset3
118458	8	404699	5	NULL	NULL	0	NULL	proinflammatory cytokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidative stress possibly via the modification of cysteine residues activates multiple stress kinase pathways and transcription factors nuclear factor-kappaB and activator protein-1 , which differentially regulate the genes for proinflammatory cytokines as well as the protective antioxidant genes .
	manualset3
118459	9	404699	5	NULL	NULL	0	NULL	protective antioxidant genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxidative stress possibly via the modification of cysteine residues activates multiple stress kinase pathways and transcription factors nuclear factor-kappaB and activator protein-1 , which differentially regulate the genes for proinflammatory cytokines as well as the protective antioxidant genes .
	manualset3
118460	1	404700	5	NULL	NULL	0	NULL	Oxygen free radicals ( OFRs ) 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxygen free radicals ( OFRs ) have been suggested in the pathogenesis of Parkinson 's disease ( PD ) .
	manualset3
118464	2	404700	5	NULL	NULL	NULL	NULL	pathogenesis 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Oxygen free radicals ( OFRs ) have been suggested in the pathogenesis of Parkinson 's disease ( PD ) .
	manualset3
118465	3	404700	5	NULL	NULL	0	NULL	Parkinson 's disease ( PD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxygen free radicals ( OFRs ) have been suggested in the pathogenesis of Parkinson 's disease ( PD ) .
	manualset3
118467	1	404701	5	NULL	NULL	0	NULL	Oxygen inhibitory effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxygen inhibitory effect could occur through the oxidation of LDH essential free sulfhydryl groups .
	manualset3
118468	2	404701	5	NULL	NULL	0	NULL	oxidation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxygen inhibitory effect could occur through the oxidation of LDH essential free sulfhydryl groups .
	manualset3
118471	3	404701	5	NULL	NULL	0	NULL	LDH essential free sulfhydryl groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxygen inhibitory effect could occur through the oxidation of LDH essential free sulfhydryl groups .
	manualset3
118474	1	404702	5	NULL	NULL	0	NULL	Oxygen insufflation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxygen insufflation can be delivered through an intranasal tube .
	manualset3
118476	2	404702	5	NULL	NULL	0	NULL	intranasal tube	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxygen insufflation can be delivered through an intranasal tube .
	manualset3
118480	1	404703	5	NULL	NULL	0	NULL	Oxytocin 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxytocin , a hormone involved in numerous physiologic processes , plays a central role in the mechanisms of parturition and lactation .
	manualset3
118481	2	404703	5	NULL	NULL	0	NULL	hormone 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxytocin , a hormone involved in numerous physiologic processes , plays a central role in the mechanisms of parturition and lactation .
	manualset3
118482	3	404703	5	NULL	NULL	0	NULL	numerous physiologic processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxytocin , a hormone involved in numerous physiologic processes , plays a central role in the mechanisms of parturition and lactation .
	manualset3
118483	4	404703	5	NULL	NULL	0	NULL	central role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxytocin , a hormone involved in numerous physiologic processes , plays a central role in the mechanisms of parturition and lactation .
	manualset3
118484	5	404703	5	NULL	NULL	0	NULL	mechanisms 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxytocin , a hormone involved in numerous physiologic processes , plays a central role in the mechanisms of parturition and lactation .
	manualset3
118486	6	404703	5	NULL	NULL	0	NULL	parturition 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxytocin , a hormone involved in numerous physiologic processes , plays a central role in the mechanisms of parturition and lactation .
	manualset3
118488	7	404703	5	NULL	NULL	0	NULL	lactation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Oxytocin , a hormone involved in numerous physiologic processes , plays a central role in the mechanisms of parturition and lactation .
	manualset3
118492	1	404704	5	NULL	NULL	0	NULL	P-ADC 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	P-ADC is the one showing a more characteristic and exclusive genetic mark , followed by CR-ADC .
	manualset3
118493	2	404704	5	NULL	NULL	NULL	NULL	characteristic and exclusive genetic mark	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	P-ADC is the one showing a more characteristic and exclusive genetic mark , followed by CR-ADC .
	manualset3
118494	3	404704	5	NULL	NULL	0	NULL	CR-ADC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	P-ADC is the one showing a more characteristic and exclusive genetic mark , followed by CR-ADC .
	manualset3
118501	1	404705	5	NULL	NULL	0	NULL	P-LPS	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	P-LPS ( 1 to 10 micrograms/ml ) and E-LPS ( 100 micrograms/ml ) markedly stimulated the expression of IL-6 and IL-8 mRNAs compared with the control .
	manualset3
118502	2	404705	5	NULL	NULL	0	NULL	1 to 10 micrograms/ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	P-LPS ( 1 to 10 micrograms/ml ) and E-LPS ( 100 micrograms/ml ) markedly stimulated the expression of IL-6 and IL-8 mRNAs compared with the control .
	manualset3
118503	3	404705	5	NULL	NULL	0	NULL	E-LPS	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	P-LPS ( 1 to 10 micrograms/ml ) and E-LPS ( 100 micrograms/ml ) markedly stimulated the expression of IL-6 and IL-8 mRNAs compared with the control .
	manualset3
118504	4	404705	5	NULL	NULL	0	NULL	100 micrograms/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	P-LPS ( 1 to 10 micrograms/ml ) and E-LPS ( 100 micrograms/ml ) markedly stimulated the expression of IL-6 and IL-8 mRNAs compared with the control .
	manualset3
118508	5	404705	5	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	P-LPS ( 1 to 10 micrograms/ml ) and E-LPS ( 100 micrograms/ml ) markedly stimulated the expression of IL-6 and IL-8 mRNAs compared with the control .
	manualset3
118510	6	404705	5	NULL	NULL	0	NULL	IL-6 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	P-LPS ( 1 to 10 micrograms/ml ) and E-LPS ( 100 micrograms/ml ) markedly stimulated the expression of IL-6 and IL-8 mRNAs compared with the control .
	manualset3
118512	7	404705	5	NULL	NULL	0	NULL	 IL-8 mRNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	P-LPS ( 1 to 10 micrograms/ml ) and E-LPS ( 100 micrograms/ml ) markedly stimulated the expression of IL-6 and IL-8 mRNAs compared with the control .
	manualset3
118513	8	404705	5	NULL	NULL	0	NULL	control 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	P-LPS ( 1 to 10 micrograms/ml ) and E-LPS ( 100 micrograms/ml ) markedly stimulated the expression of IL-6 and IL-8 mRNAs compared with the control .
	manualset3
118514	1	404706	5	NULL	NULL	0	NULL	P ( p )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	P ( p ) is sensed by a pressure sensor integrated into the magnetic clamp .
	manualset3
118515	2	404706	5	NULL	NULL	0	NULL	pressure sensor	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	P ( p ) is sensed by a pressure sensor integrated into the magnetic clamp .
	manualset3
118516	3	404706	5	NULL	NULL	0	NULL	magnetic clamp	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	P ( p ) is sensed by a pressure sensor integrated into the magnetic clamp .
	manualset3
118517	1	404707	5	NULL	NULL	0	NULL	P311 - / - mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	P311 - / - mice showed normal heat and mechanical sensitivity , as well as normal formalin-induced inflammatory pain .
	manualset3
118518	2	404707	5	NULL	NULL	0	NULL	normal heat	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	P311 - / - mice showed normal heat and mechanical sensitivity , as well as normal formalin-induced inflammatory pain .
	manualset3
118519	3	404707	5	NULL	NULL	0	NULL	mechanical sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	P311 - / - mice showed normal heat and mechanical sensitivity , as well as normal formalin-induced inflammatory pain .
	manualset3
118520	4	404707	5	NULL	NULL	0	NULL	normal formalin-induced inflammatory pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	P311 - / - mice showed normal heat and mechanical sensitivity , as well as normal formalin-induced inflammatory pain .
	manualset3
118522	1	404708	5	NULL	NULL	0	NULL	P44 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	P44 should be stabilized by intrahelical hydrogen bonds , interhelical disulfide and salt bridges , and interior hydrophobic interactions .
	manualset3
118524	2	404708	5	NULL	NULL	0	NULL	intrahelical hydrogen bonds	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	P44 should be stabilized by intrahelical hydrogen bonds , interhelical disulfide and salt bridges , and interior hydrophobic interactions .
	manualset3
118526	3	404708	5	NULL	NULL	0	NULL	interhelical disulfide and salt bridges	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	P44 should be stabilized by intrahelical hydrogen bonds , interhelical disulfide and salt bridges , and interior hydrophobic interactions .
	manualset3
118528	4	404708	5	NULL	NULL	0	NULL	interior hydrophobic interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	P44 should be stabilized by intrahelical hydrogen bonds , interhelical disulfide and salt bridges , and interior hydrophobic interactions .
	manualset3
118529	1	404709	5	NULL	NULL	0	NULL	PA-induced apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PA-induced apoptosis and mitochondrial dysfunction in a dose-dependent manner as evaluated by DNA fragmentation assay and depolarization of the mitochondrial membrane , respectively .
	manualset3
118530	2	404709	5	NULL	NULL	0	NULL	mitochondrial dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	PA-induced apoptosis and mitochondrial dysfunction in a dose-dependent manner as evaluated by DNA fragmentation assay and depolarization of the mitochondrial membrane , respectively .
	manualset3
118531	3	404709	5	NULL	NULL	0	NULL	dose-dependent manner	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PA-induced apoptosis and mitochondrial dysfunction in a dose-dependent manner as evaluated by DNA fragmentation assay and depolarization of the mitochondrial membrane , respectively .
	manualset3
118533	4	404709	5	NULL	NULL	0	NULL	DNA fragmentation assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	PA-induced apoptosis and mitochondrial dysfunction in a dose-dependent manner as evaluated by DNA fragmentation assay and depolarization of the mitochondrial membrane , respectively .
	manualset3
118535	5	404709	5	NULL	NULL	NULL	NULL	depolarization 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	PA-induced apoptosis and mitochondrial dysfunction in a dose-dependent manner as evaluated by DNA fragmentation assay and depolarization of the mitochondrial membrane , respectively .
	manualset3
118537	6	404709	5	NULL	NULL	0	NULL	mitochondrial membrane 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	PA-induced apoptosis and mitochondrial dysfunction in a dose-dependent manner as evaluated by DNA fragmentation assay and depolarization of the mitochondrial membrane , respectively .
	manualset3
118545	1	404710	5	NULL	NULL	NULL	NULL	PACAPs	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	PACAPs and VIP interact with the same affinity and stimulate adenylate cyclase activity with the same efficacy and potency on the VIP receptors , but PACAPs act also on a more selective PACAP receptor that also recognizes VIP but with a 100 - to 1 , 000-fold lower affinity .
	manualset3
118547	2	404710	5	NULL	NULL	NULL	NULL	VIP 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	PACAPs and VIP interact with the same affinity and stimulate adenylate cyclase activity with the same efficacy and potency on the VIP receptors , but PACAPs act also on a more selective PACAP receptor that also recognizes VIP but with a 100 - to 1 , 000-fold lower affinity .
	manualset3
118550	3	404710	5	NULL	NULL	0	NULL	affinity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PACAPs and VIP interact with the same affinity and stimulate adenylate cyclase activity with the same efficacy and potency on the VIP receptors , but PACAPs act also on a more selective PACAP receptor that also recognizes VIP but with a 100 - to 1 , 000-fold lower affinity .
	manualset3
118551	4	404710	5	NULL	NULL	0	NULL	adenylate cyclase activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PACAPs and VIP interact with the same affinity and stimulate adenylate cyclase activity with the same efficacy and potency on the VIP receptors , but PACAPs act also on a more selective PACAP receptor that also recognizes VIP but with a 100 - to 1 , 000-fold lower affinity .
	manualset3
118552	5	404710	5	NULL	NULL	0	NULL	efficacy 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PACAPs and VIP interact with the same affinity and stimulate adenylate cyclase activity with the same efficacy and potency on the VIP receptors , but PACAPs act also on a more selective PACAP receptor that also recognizes VIP but with a 100 - to 1 , 000-fold lower affinity .
	manualset3
118553	6	404710	5	NULL	NULL	0	NULL	potency 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PACAPs and VIP interact with the same affinity and stimulate adenylate cyclase activity with the same efficacy and potency on the VIP receptors , but PACAPs act also on a more selective PACAP receptor that also recognizes VIP but with a 100 - to 1 , 000-fold lower affinity .
	manualset3
118554	7	404710	5	NULL	NULL	0	NULL	VIP receptors 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PACAPs and VIP interact with the same affinity and stimulate adenylate cyclase activity with the same efficacy and potency on the VIP receptors , but PACAPs act also on a more selective PACAP receptor that also recognizes VIP but with a 100 - to 1 , 000-fold lower affinity .
	manualset3
118555	8	404710	5	NULL	NULL	0	NULL	PACAPs 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PACAPs and VIP interact with the same affinity and stimulate adenylate cyclase activity with the same efficacy and potency on the VIP receptors , but PACAPs act also on a more selective PACAP receptor that also recognizes VIP but with a 100 - to 1 , 000-fold lower affinity .
	manualset3
118556	9	404710	5	NULL	NULL	0	NULL	PACAP receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PACAPs and VIP interact with the same affinity and stimulate adenylate cyclase activity with the same efficacy and potency on the VIP receptors , but PACAPs act also on a more selective PACAP receptor that also recognizes VIP but with a 100 - to 1 , 000-fold lower affinity .
	manualset3
118557	10	404710	5	NULL	NULL	0	NULL	VIP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PACAPs and VIP interact with the same affinity and stimulate adenylate cyclase activity with the same efficacy and potency on the VIP receptors , but PACAPs act also on a more selective PACAP receptor that also recognizes VIP but with a 100 - to 1 , 000-fold lower affinity .
	manualset3
118558	11	404710	5	NULL	NULL	0	NULL	100 - to 1 , 000-fold lower affinity	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	PACAPs and VIP interact with the same affinity and stimulate adenylate cyclase activity with the same efficacy and potency on the VIP receptors , but PACAPs act also on a more selective PACAP receptor that also recognizes VIP but with a 100 - to 1 , 000-fold lower affinity .
	manualset3
118997	1	404711	5	NULL	NULL	0	NULL	PAHs	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	PAHs were detected in all of the samples , with total concentrations between 390 and 6390 ng/g dry weight for the 27 PAHs analyzed and from 310 to 5120 ng/g dry weight for the sum of the 10 PAHs considered in the draft European Union directive .
	manualset3
118998	2	404711	5	NULL	NULL	0	NULL	samples	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	PAHs were detected in all of the samples , with total concentrations between 390 and 6390 ng/g dry weight for the 27 PAHs analyzed and from 310 to 5120 ng/g dry weight for the sum of the 10 PAHs considered in the draft European Union directive .
	manualset3
118999	3	404711	5	NULL	NULL	0	NULL	total concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PAHs were detected in all of the samples , with total concentrations between 390 and 6390 ng/g dry weight for the 27 PAHs analyzed and from 310 to 5120 ng/g dry weight for the sum of the 10 PAHs considered in the draft European Union directive .
	manualset3
119000	4	404711	5	NULL	NULL	0	NULL	390 and 6390 ng/g dry weight 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	PAHs were detected in all of the samples , with total concentrations between 390 and 6390 ng/g dry weight for the 27 PAHs analyzed and from 310 to 5120 ng/g dry weight for the sum of the 10 PAHs considered in the draft European Union directive .
	manualset3
119001	5	404711	5	NULL	NULL	0	NULL	27 PAHs	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	PAHs were detected in all of the samples , with total concentrations between 390 and 6390 ng/g dry weight for the 27 PAHs analyzed and from 310 to 5120 ng/g dry weight for the sum of the 10 PAHs considered in the draft European Union directive .
	manualset3
119002	6	404711	5	NULL	NULL	0	NULL	310 to 5120 ng/g dry weight	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	PAHs were detected in all of the samples , with total concentrations between 390 and 6390 ng/g dry weight for the 27 PAHs analyzed and from 310 to 5120 ng/g dry weight for the sum of the 10 PAHs considered in the draft European Union directive .
	manualset3
119003	7	404711	5	NULL	NULL	0	NULL	sum	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PAHs were detected in all of the samples , with total concentrations between 390 and 6390 ng/g dry weight for the 27 PAHs analyzed and from 310 to 5120 ng/g dry weight for the sum of the 10 PAHs considered in the draft European Union directive .
	manualset3
119004	8	404711	5	NULL	NULL	0	NULL	10 PAHs	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	PAHs were detected in all of the samples , with total concentrations between 390 and 6390 ng/g dry weight for the 27 PAHs analyzed and from 310 to 5120 ng/g dry weight for the sum of the 10 PAHs considered in the draft European Union directive .
	manualset3
119005	9	404711	5	NULL	NULL	0	NULL	draft European Union directive	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	PAHs were detected in all of the samples , with total concentrations between 390 and 6390 ng/g dry weight for the 27 PAHs analyzed and from 310 to 5120 ng/g dry weight for the sum of the 10 PAHs considered in the draft European Union directive .
	manualset3
119006	1	404712	5	NULL	NULL	0	NULL	PAI-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PAI-1 : cardiac friend or foe ?
	manualset3
119007	2	404712	5	NULL	NULL	NULL	NULL	cardiac friend	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	PAI-1 : cardiac friend or foe ?
	manualset3
119008	3	404712	5	NULL	NULL	0	NULL	foe	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	PAI-1 : cardiac friend or foe ?
	manualset3
119009	1	404713	5	NULL	NULL	0	NULL	PAR-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PAR-1 is regulated developmentally in the eye , with a decrease from P1 , P9 , to P16 , whereas levels for PAR-2 , PAR-3 , and PAR-4 remain unchanged throughout .
	manualset3
119010	2	404713	5	NULL	NULL	0	NULL	eye	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	PAR-1 is regulated developmentally in the eye , with a decrease from P1 , P9 , to P16 , whereas levels for PAR-2 , PAR-3 , and PAR-4 remain unchanged throughout .
	manualset3
119011	3	404713	5	NULL	NULL	0	NULL	P1	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	PAR-1 is regulated developmentally in the eye , with a decrease from P1 , P9 , to P16 , whereas levels for PAR-2 , PAR-3 , and PAR-4 remain unchanged throughout .
	manualset3
119012	4	404713	5	NULL	NULL	0	NULL	P9	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	PAR-1 is regulated developmentally in the eye , with a decrease from P1 , P9 , to P16 , whereas levels for PAR-2 , PAR-3 , and PAR-4 remain unchanged throughout .
	manualset3
119013	5	404713	5	NULL	NULL	0	NULL	P16	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	PAR-1 is regulated developmentally in the eye , with a decrease from P1 , P9 , to P16 , whereas levels for PAR-2 , PAR-3 , and PAR-4 remain unchanged throughout .
	manualset3
119014	6	404713	5	NULL	NULL	0	NULL	levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PAR-1 is regulated developmentally in the eye , with a decrease from P1 , P9 , to P16 , whereas levels for PAR-2 , PAR-3 , and PAR-4 remain unchanged throughout .
	manualset3
119015	7	404713	5	NULL	NULL	0	NULL	PAR-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PAR-1 is regulated developmentally in the eye , with a decrease from P1 , P9 , to P16 , whereas levels for PAR-2 , PAR-3 , and PAR-4 remain unchanged throughout .
	manualset3
119016	8	404713	5	NULL	NULL	0	NULL	PAR-3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PAR-1 is regulated developmentally in the eye , with a decrease from P1 , P9 , to P16 , whereas levels for PAR-2 , PAR-3 , and PAR-4 remain unchanged throughout .
	manualset3
119017	9	404713	5	NULL	NULL	0	NULL	PAR-4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PAR-1 is regulated developmentally in the eye , with a decrease from P1 , P9 , to P16 , whereas levels for PAR-2 , PAR-3 , and PAR-4 remain unchanged throughout .
	manualset3
119018	1	404714	5	NULL	NULL	0	NULL	PBCA nanoparticles	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	PBCA nanoparticles do not induce nonspecific BBB disruption , but collaborate with plasma apolipoprotein E to facilitate BBB crossing .
	manualset3
119019	2	404714	5	NULL	NULL	0	NULL	nonspecific BBB disruption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PBCA nanoparticles do not induce nonspecific BBB disruption , but collaborate with plasma apolipoprotein E to facilitate BBB crossing .
	manualset3
119020	3	404714	5	NULL	NULL	0	NULL	plasma apolipoprotein E	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PBCA nanoparticles do not induce nonspecific BBB disruption , but collaborate with plasma apolipoprotein E to facilitate BBB crossing .
	manualset3
119021	4	404714	5	NULL	NULL	0	NULL	BBB crossing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PBCA nanoparticles do not induce nonspecific BBB disruption , but collaborate with plasma apolipoprotein E to facilitate BBB crossing .
	manualset3
119022	1	404715	5	NULL	NULL	0	NULL	PBF	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	PBF and systemic blood pressure dropped significantly after LPS administration .
	manualset3
119023	2	404715	5	NULL	NULL	0	NULL	systemic blood pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PBF and systemic blood pressure dropped significantly after LPS administration .
	manualset3
119024	3	404715	5	NULL	NULL	0	NULL	LPS administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	PBF and systemic blood pressure dropped significantly after LPS administration .
	manualset3
119025	1	404716	5	NULL	NULL	0	NULL	PC12EN	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	PC12EN lacked receptors for EGF and both the p75 and trk NGF receptors , while FGF receptor expression was maintained .
	manualset3
119026	2	404716	5	NULL	NULL	0	NULL	receptors for EGF	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	PC12EN lacked receptors for EGF and both the p75 and trk NGF receptors , while FGF receptor expression was maintained .
	manualset3
119027	3	404716	5	NULL	NULL	0	NULL	p75 receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PC12EN lacked receptors for EGF and both the p75 and trk NGF receptors , while FGF receptor expression was maintained .
	manualset3
119028	4	404716	5	NULL	NULL	0	NULL	trk NGF receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PC12EN lacked receptors for EGF and both the p75 and trk NGF receptors , while FGF receptor expression was maintained .
	manualset3
119029	5	404716	5	NULL	NULL	0	NULL	FGF receptor expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PC12EN lacked receptors for EGF and both the p75 and trk NGF receptors , while FGF receptor expression was maintained .
	manualset3
119030	1	404717	5	NULL	NULL	0	NULL	PC3-PIP cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	PC3-PIP cells are derived from PC3 that have been transduced with the gene for PSMA .
	manualset3
119031	2	404717	5	NULL	NULL	0	NULL	PC3	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	PC3-PIP cells are derived from PC3 that have been transduced with the gene for PSMA .
	manualset3
119032	3	404717	5	NULL	NULL	0	NULL	gene for PSMA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	PC3-PIP cells are derived from PC3 that have been transduced with the gene for PSMA .
	manualset3
119033	1	404718	5	NULL	NULL	0	NULL	PCA	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PCA was measured by recalcification time of normal plasma with the cell lysate , XAA and PlgAA was measured by chromogenic substrate .
	manualset3
119034	2	404718	5	NULL	NULL	0	NULL	recalcification time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	PCA was measured by recalcification time of normal plasma with the cell lysate , XAA and PlgAA was measured by chromogenic substrate .
	manualset3
119035	3	404718	5	NULL	NULL	0	NULL	normal plasma	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	PCA was measured by recalcification time of normal plasma with the cell lysate , XAA and PlgAA was measured by chromogenic substrate .
	manualset3
119036	4	404718	5	NULL	NULL	0	NULL	cell lysate	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	PCA was measured by recalcification time of normal plasma with the cell lysate , XAA and PlgAA was measured by chromogenic substrate .
	manualset3
119037	5	404718	5	NULL	NULL	0	NULL	XAA	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PCA was measured by recalcification time of normal plasma with the cell lysate , XAA and PlgAA was measured by chromogenic substrate .
	manualset3
119038	6	404718	5	NULL	NULL	0	NULL	PlgAA	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PCA was measured by recalcification time of normal plasma with the cell lysate , XAA and PlgAA was measured by chromogenic substrate .
	manualset3
119039	7	404718	5	NULL	NULL	0	NULL	chromogenic substrate	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	PCA was measured by recalcification time of normal plasma with the cell lysate , XAA and PlgAA was measured by chromogenic substrate .
	manualset3
119040	1	404719	5	NULL	NULL	0	NULL	PCC 7002	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	PCC 7002 exhibited glucosyl-phosphoglycerate synthase ( GpgS ) activity , and GpgS is a key enzyme of GGA synthesis .
	manualset3
119041	2	404719	5	NULL	NULL	0	NULL	glucosyl-phosphoglycerate synthase ( GpgS ) activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PCC 7002 exhibited glucosyl-phosphoglycerate synthase ( GpgS ) activity , and GpgS is a key enzyme of GGA synthesis .
	manualset3
119042	3	404719	5	NULL	NULL	0	NULL	GpgS	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PCC 7002 exhibited glucosyl-phosphoglycerate synthase ( GpgS ) activity , and GpgS is a key enzyme of GGA synthesis .
	manualset3
119043	4	404719	5	NULL	NULL	0	NULL	key enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PCC 7002 exhibited glucosyl-phosphoglycerate synthase ( GpgS ) activity , and GpgS is a key enzyme of GGA synthesis .
	manualset3
119044	5	404719	5	NULL	NULL	0	NULL	GGA synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PCC 7002 exhibited glucosyl-phosphoglycerate synthase ( GpgS ) activity , and GpgS is a key enzyme of GGA synthesis .
	manualset3
119045	1	404720	5	NULL	NULL	0	NULL	PCR amplification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	PCR amplification of genes coding bacteriocins and determination of their nucleotide sequence , and the use of specific antipeptide bacteriocin antibodies and a noncompetitive indirect enzyme-linked immunosorbent assay , permitted characterization of enterococci coding that described bacteriocins and their expression .
	manualset3
119046	2	404720	5	NULL	NULL	0	NULL	genes coding bacteriocins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	PCR amplification of genes coding bacteriocins and determination of their nucleotide sequence , and the use of specific antipeptide bacteriocin antibodies and a noncompetitive indirect enzyme-linked immunosorbent assay , permitted characterization of enterococci coding that described bacteriocins and their expression .
	manualset3
119047	3	404720	5	NULL	NULL	0	NULL	determination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PCR amplification of genes coding bacteriocins and determination of their nucleotide sequence , and the use of specific antipeptide bacteriocin antibodies and a noncompetitive indirect enzyme-linked immunosorbent assay , permitted characterization of enterococci coding that described bacteriocins and their expression .
	manualset3
119048	4	404720	5	NULL	NULL	0	NULL	nucleotide sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	PCR amplification of genes coding bacteriocins and determination of their nucleotide sequence , and the use of specific antipeptide bacteriocin antibodies and a noncompetitive indirect enzyme-linked immunosorbent assay , permitted characterization of enterococci coding that described bacteriocins and their expression .
	manualset3
119049	5	404720	5	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PCR amplification of genes coding bacteriocins and determination of their nucleotide sequence , and the use of specific antipeptide bacteriocin antibodies and a noncompetitive indirect enzyme-linked immunosorbent assay , permitted characterization of enterococci coding that described bacteriocins and their expression .
	manualset3
119050	6	404720	5	NULL	NULL	0	NULL	specific antipeptide bacteriocin antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	PCR amplification of genes coding bacteriocins and determination of their nucleotide sequence , and the use of specific antipeptide bacteriocin antibodies and a noncompetitive indirect enzyme-linked immunosorbent assay , permitted characterization of enterococci coding that described bacteriocins and their expression .
	manualset3
119051	7	404720	5	NULL	NULL	0	NULL	noncompetitive indirect enzyme-linked immunosorbent assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	PCR amplification of genes coding bacteriocins and determination of their nucleotide sequence , and the use of specific antipeptide bacteriocin antibodies and a noncompetitive indirect enzyme-linked immunosorbent assay , permitted characterization of enterococci coding that described bacteriocins and their expression .
	manualset3
119052	8	404720	5	NULL	NULL	NULL	NULL	characterization	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	PCR amplification of genes coding bacteriocins and determination of their nucleotide sequence , and the use of specific antipeptide bacteriocin antibodies and a noncompetitive indirect enzyme-linked immunosorbent assay , permitted characterization of enterococci coding that described bacteriocins and their expression .
	manualset3
119053	9	404720	5	NULL	NULL	0	NULL	enterococci	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	PCR amplification of genes coding bacteriocins and determination of their nucleotide sequence , and the use of specific antipeptide bacteriocin antibodies and a noncompetitive indirect enzyme-linked immunosorbent assay , permitted characterization of enterococci coding that described bacteriocins and their expression .
	manualset3
119054	10	404720	5	NULL	NULL	0	NULL	bacteriocins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PCR amplification of genes coding bacteriocins and determination of their nucleotide sequence , and the use of specific antipeptide bacteriocin antibodies and a noncompetitive indirect enzyme-linked immunosorbent assay , permitted characterization of enterococci coding that described bacteriocins and their expression .
	manualset3
119055	11	404720	5	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PCR amplification of genes coding bacteriocins and determination of their nucleotide sequence , and the use of specific antipeptide bacteriocin antibodies and a noncompetitive indirect enzyme-linked immunosorbent assay , permitted characterization of enterococci coding that described bacteriocins and their expression .
	manualset3
119056	1	404721	5	NULL	NULL	0	NULL	PCR amplification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	PCR amplification with these primers generated a product of the expected size directly from the crude feces of HPV-infected shrimp but not from the feces of specific pathogen-free ( SPF ) shrimp .
	manualset3
119057	2	404721	5	NULL	NULL	0	NULL	primers	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	PCR amplification with these primers generated a product of the expected size directly from the crude feces of HPV-infected shrimp but not from the feces of specific pathogen-free ( SPF ) shrimp .
	manualset3
119058	3	404721	5	NULL	NULL	0	NULL	product	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	PCR amplification with these primers generated a product of the expected size directly from the crude feces of HPV-infected shrimp but not from the feces of specific pathogen-free ( SPF ) shrimp .
	manualset3
119059	4	404721	5	NULL	NULL	0	NULL	expected size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PCR amplification with these primers generated a product of the expected size directly from the crude feces of HPV-infected shrimp but not from the feces of specific pathogen-free ( SPF ) shrimp .
	manualset3
119060	5	404721	5	NULL	NULL	0	NULL	crude feces	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	PCR amplification with these primers generated a product of the expected size directly from the crude feces of HPV-infected shrimp but not from the feces of specific pathogen-free ( SPF ) shrimp .
	manualset3
119061	6	404721	5	NULL	NULL	0	NULL	HPV-infected shrimp	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	PCR amplification with these primers generated a product of the expected size directly from the crude feces of HPV-infected shrimp but not from the feces of specific pathogen-free ( SPF ) shrimp .
	manualset3
119062	7	404721	5	NULL	NULL	0	NULL	feces	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	PCR amplification with these primers generated a product of the expected size directly from the crude feces of HPV-infected shrimp but not from the feces of specific pathogen-free ( SPF ) shrimp .
	manualset3
119063	8	404721	5	NULL	NULL	0	NULL	specific pathogen-free ( SPF ) shrimp	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	PCR amplification with these primers generated a product of the expected size directly from the crude feces of HPV-infected shrimp but not from the feces of specific pathogen-free ( SPF ) shrimp .
	manualset3
119064	1	404722	5	NULL	NULL	0	NULL	follow-up enquiry	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A follow-up enquiry was carried out after two years on 54 patients who had earlier participated in a controlled experiment on home-care through a community nurse in Bangalore .
	manualset3
119065	2	404722	5	NULL	NULL	0	NULL	two years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A follow-up enquiry was carried out after two years on 54 patients who had earlier participated in a controlled experiment on home-care through a community nurse in Bangalore .
	manualset3
119066	3	404722	5	NULL	NULL	0	NULL	54 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A follow-up enquiry was carried out after two years on 54 patients who had earlier participated in a controlled experiment on home-care through a community nurse in Bangalore .
	manualset3
119067	4	404722	5	NULL	NULL	0	NULL	 controlled experiment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A follow-up enquiry was carried out after two years on 54 patients who had earlier participated in a controlled experiment on home-care through a community nurse in Bangalore .
	manualset3
119068	5	404722	5	NULL	NULL	0	NULL	home-care	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A follow-up enquiry was carried out after two years on 54 patients who had earlier participated in a controlled experiment on home-care through a community nurse in Bangalore .
	manualset3
119069	6	404722	5	NULL	NULL	0	NULL	community nurse	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A follow-up enquiry was carried out after two years on 54 patients who had earlier participated in a controlled experiment on home-care through a community nurse in Bangalore .
	manualset3
119070	7	404722	5	NULL	NULL	0	NULL	Bangalore	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A follow-up enquiry was carried out after two years on 54 patients who had earlier participated in a controlled experiment on home-care through a community nurse in Bangalore .
	manualset3
119071	1	404723	5	NULL	NULL	0	NULL	PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	PCR and reverse transcriptase ( RT ) PCR were used to amplify 16S ribosomal DNA ( rDNA ) and 16S rRNA , respectively , and the products were subjected to denaturing gradient gel electrophoresis ( DGGE ) .
	manualset3
119072	2	404723	5	NULL	NULL	0	NULL	reverse transcriptase ( RT ) PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	PCR and reverse transcriptase ( RT ) PCR were used to amplify 16S ribosomal DNA ( rDNA ) and 16S rRNA , respectively , and the products were subjected to denaturing gradient gel electrophoresis ( DGGE ) .
	manualset3
119073	3	404723	5	NULL	NULL	0	NULL	16S ribosomal DNA ( rDNA ) 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	PCR and reverse transcriptase ( RT ) PCR were used to amplify 16S ribosomal DNA ( rDNA ) and 16S rRNA , respectively , and the products were subjected to denaturing gradient gel electrophoresis ( DGGE ) .
	manualset3
119074	4	404723	5	NULL	NULL	0	NULL	16S rRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	PCR and reverse transcriptase ( RT ) PCR were used to amplify 16S ribosomal DNA ( rDNA ) and 16S rRNA , respectively , and the products were subjected to denaturing gradient gel electrophoresis ( DGGE ) .
	manualset3
119075	5	404723	5	NULL	NULL	0	NULL	products	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	PCR and reverse transcriptase ( RT ) PCR were used to amplify 16S ribosomal DNA ( rDNA ) and 16S rRNA , respectively , and the products were subjected to denaturing gradient gel electrophoresis ( DGGE ) .
	manualset3
119076	6	404723	5	NULL	NULL	0	NULL	denaturing gradient gel electrophoresis ( DGGE )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	PCR and reverse transcriptase ( RT ) PCR were used to amplify 16S ribosomal DNA ( rDNA ) and 16S rRNA , respectively , and the products were subjected to denaturing gradient gel electrophoresis ( DGGE ) .
	manualset3
119077	1	404724	5	NULL	NULL	0	NULL	PCR results	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	PCR results showed that the pleiotropic virulence regulator plcR was presented in 17 B. cereus group strains .
	manualset3
119078	2	404724	5	NULL	NULL	0	NULL	pleiotropic virulence regulator plcR	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	PCR results showed that the pleiotropic virulence regulator plcR was presented in 17 B. cereus group strains .
	manualset3
119079	3	404724	5	NULL	NULL	0	NULL	17 B. cereus group strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	PCR results showed that the pleiotropic virulence regulator plcR was presented in 17 B. cereus group strains .
	manualset3
119080	1	404725	5	NULL	NULL	0	NULL	PCSK4-null sperm display	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PCSK4-null sperm display enhanced protein tyrosine phosphorylation and ADAM2 proteolytic processing during in vitro capacitation .
	manualset3
119081	2	404725	5	NULL	NULL	0	NULL	protein tyrosine phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PCSK4-null sperm display enhanced protein tyrosine phosphorylation and ADAM2 proteolytic processing during in vitro capacitation .
	manualset3
119082	3	404725	5	NULL	NULL	0	NULL	ADAM2 proteolytic processing	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PCSK4-null sperm display enhanced protein tyrosine phosphorylation and ADAM2 proteolytic processing during in vitro capacitation .
	manualset3
119083	4	404725	5	NULL	NULL	0	NULL	in vitro capacitation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	PCSK4-null sperm display enhanced protein tyrosine phosphorylation and ADAM2 proteolytic processing during in vitro capacitation .
	manualset3
119084	1	404726	5	NULL	NULL	0	NULL	PD	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	PD and DQ are determined simultaneously with a diode array UV absorbance detector .
	manualset3
119085	2	404726	5	NULL	NULL	0	NULL	DQ	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	PD and DQ are determined simultaneously with a diode array UV absorbance detector .
	manualset3
119086	3	404726	5	NULL	NULL	0	NULL	diode array UV absorbance detector	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	PD and DQ are determined simultaneously with a diode array UV absorbance detector .
	manualset3
119087	1	404727	5	NULL	NULL	0	NULL	PDBu	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	PDBu ( 0.01 and 0.1 microM ) elevated resting tension of the veins more effectively than TPA and mezerein .
	manualset3
119088	2	404727	5	NULL	NULL	0	NULL	 0.01 and 0.1 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	PDBu ( 0.01 and 0.1 microM ) elevated resting tension of the veins more effectively than TPA and mezerein .
	manualset3
119089	3	404727	5	NULL	NULL	0	NULL	tension	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PDBu ( 0.01 and 0.1 microM ) elevated resting tension of the veins more effectively than TPA and mezerein .
	manualset3
119090	4	404727	5	NULL	NULL	0	NULL	veins	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	PDBu ( 0.01 and 0.1 microM ) elevated resting tension of the veins more effectively than TPA and mezerein .
	manualset3
119091	5	404727	5	NULL	NULL	0	NULL	TPA	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	PDBu ( 0.01 and 0.1 microM ) elevated resting tension of the veins more effectively than TPA and mezerein .
	manualset3
119092	6	404727	5	NULL	NULL	0	NULL	mezerein	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	PDBu ( 0.01 and 0.1 microM ) elevated resting tension of the veins more effectively than TPA and mezerein .
	manualset3
119093	1	404728	5	NULL	NULL	0	NULL	PDBu	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	PDBu at concentrations higher than 100 nmol/L inhibited the positive inotropic effects of Bay K 8644 and isoproterenol , and decreased the basal force of contraction in a concentration-dependent manner to a similar extent .
	manualset3
119094	2	404728	5	NULL	NULL	0	NULL	concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PDBu at concentrations higher than 100 nmol/L inhibited the positive inotropic effects of Bay K 8644 and isoproterenol , and decreased the basal force of contraction in a concentration-dependent manner to a similar extent .
	manualset3
119095	3	404728	5	NULL	NULL	0	NULL	100 nmol/L 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	PDBu at concentrations higher than 100 nmol/L inhibited the positive inotropic effects of Bay K 8644 and isoproterenol , and decreased the basal force of contraction in a concentration-dependent manner to a similar extent .
	manualset3
119096	4	404728	5	NULL	NULL	0	NULL	positive inotropic effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PDBu at concentrations higher than 100 nmol/L inhibited the positive inotropic effects of Bay K 8644 and isoproterenol , and decreased the basal force of contraction in a concentration-dependent manner to a similar extent .
	manualset3
119097	5	404728	5	NULL	NULL	0	NULL	Bay K 8644	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	PDBu at concentrations higher than 100 nmol/L inhibited the positive inotropic effects of Bay K 8644 and isoproterenol , and decreased the basal force of contraction in a concentration-dependent manner to a similar extent .
	manualset3
119098	6	404728	5	NULL	NULL	0	NULL	isoproterenol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	PDBu at concentrations higher than 100 nmol/L inhibited the positive inotropic effects of Bay K 8644 and isoproterenol , and decreased the basal force of contraction in a concentration-dependent manner to a similar extent .
	manualset3
119099	7	404728	5	NULL	NULL	0	NULL	basal force	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PDBu at concentrations higher than 100 nmol/L inhibited the positive inotropic effects of Bay K 8644 and isoproterenol , and decreased the basal force of contraction in a concentration-dependent manner to a similar extent .
	manualset3
119100	8	404728	5	NULL	NULL	0	NULL	contraction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PDBu at concentrations higher than 100 nmol/L inhibited the positive inotropic effects of Bay K 8644 and isoproterenol , and decreased the basal force of contraction in a concentration-dependent manner to a similar extent .
	manualset3
119101	9	404728	5	NULL	NULL	0	NULL	concentration-dependent manner	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PDBu at concentrations higher than 100 nmol/L inhibited the positive inotropic effects of Bay K 8644 and isoproterenol , and decreased the basal force of contraction in a concentration-dependent manner to a similar extent .
	manualset3
119102	1	404729	5	NULL	NULL	0	NULL	PDCD6 protein expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PDCD6 protein expression was examined in 169 advanced gastric cancer specimens by immunohistochemistry and then correlated with clinicopathologic parameters .
	manualset3
119103	2	404729	5	NULL	NULL	0	NULL	169 advanced gastric cancer specimens	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	PDCD6 protein expression was examined in 169 advanced gastric cancer specimens by immunohistochemistry and then correlated with clinicopathologic parameters .
	manualset3
119104	3	404729	5	NULL	NULL	0	NULL	immunohistochemistry	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	PDCD6 protein expression was examined in 169 advanced gastric cancer specimens by immunohistochemistry and then correlated with clinicopathologic parameters .
	manualset3
119105	4	404729	5	NULL	NULL	0	NULL	clinicopathologic parameters	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	PDCD6 protein expression was examined in 169 advanced gastric cancer specimens by immunohistochemistry and then correlated with clinicopathologic parameters .
	manualset3
119106	1	404730	5	NULL	NULL	0	NULL	PDE8A immunoreactivity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PDE8A immunoreactivity was represented in the epithelial lining of the choroids plexus , the dura mater , and the neurons of the trigeminal ganglion .
	manualset3
119107	2	404730	5	NULL	NULL	0	NULL	epithelial lining	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	PDE8A immunoreactivity was represented in the epithelial lining of the choroids plexus , the dura mater , and the neurons of the trigeminal ganglion .
	manualset3
119108	3	404730	5	NULL	NULL	0	NULL	choroids plexus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	PDE8A immunoreactivity was represented in the epithelial lining of the choroids plexus , the dura mater , and the neurons of the trigeminal ganglion .
	manualset3
119109	4	404730	5	NULL	NULL	0	NULL	dura mater	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	PDE8A immunoreactivity was represented in the epithelial lining of the choroids plexus , the dura mater , and the neurons of the trigeminal ganglion .
	manualset3
119110	5	404730	5	NULL	NULL	0	NULL	neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	PDE8A immunoreactivity was represented in the epithelial lining of the choroids plexus , the dura mater , and the neurons of the trigeminal ganglion .
	manualset3
119111	6	404730	5	NULL	NULL	0	NULL	trigeminal ganglion	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	PDE8A immunoreactivity was represented in the epithelial lining of the choroids plexus , the dura mater , and the neurons of the trigeminal ganglion .
	manualset3
119112	1	404731	5	NULL	NULL	NULL	NULL	PERSPECTIVE 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	PERSPECTIVE : This article presents results of a pivotal Phase 3 study that assesses a new treatment for the management of chronic low back pain : a transdermal patch containing the opioid buprenorphine ( BTDS ) .
	manualset3
119113	2	404731	5	NULL	NULL	0	NULL	article 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	PERSPECTIVE : This article presents results of a pivotal Phase 3 study that assesses a new treatment for the management of chronic low back pain : a transdermal patch containing the opioid buprenorphine ( BTDS ) .
	manualset3
119114	3	404731	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	PERSPECTIVE : This article presents results of a pivotal Phase 3 study that assesses a new treatment for the management of chronic low back pain : a transdermal patch containing the opioid buprenorphine ( BTDS ) .
	manualset3
119115	4	404731	5	NULL	NULL	0	NULL	pivotal Phase 3 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	PERSPECTIVE : This article presents results of a pivotal Phase 3 study that assesses a new treatment for the management of chronic low back pain : a transdermal patch containing the opioid buprenorphine ( BTDS ) .
	manualset3
119116	5	404731	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	PERSPECTIVE : This article presents results of a pivotal Phase 3 study that assesses a new treatment for the management of chronic low back pain : a transdermal patch containing the opioid buprenorphine ( BTDS ) .
	manualset3
119117	6	404731	5	NULL	NULL	0	NULL	management 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	PERSPECTIVE : This article presents results of a pivotal Phase 3 study that assesses a new treatment for the management of chronic low back pain : a transdermal patch containing the opioid buprenorphine ( BTDS ) .
	manualset3
119118	7	404731	5	NULL	NULL	0	NULL	chronic low back pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	PERSPECTIVE : This article presents results of a pivotal Phase 3 study that assesses a new treatment for the management of chronic low back pain : a transdermal patch containing the opioid buprenorphine ( BTDS ) .
	manualset3
119119	8	404731	5	NULL	NULL	NULL	NULL	transdermal patch 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	PERSPECTIVE : This article presents results of a pivotal Phase 3 study that assesses a new treatment for the management of chronic low back pain : a transdermal patch containing the opioid buprenorphine ( BTDS ) .
	manualset3
119120	9	404731	5	NULL	NULL	0	NULL	opioid buprenorphine ( BTDS )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	PERSPECTIVE : This article presents results of a pivotal Phase 3 study that assesses a new treatment for the management of chronic low back pain : a transdermal patch containing the opioid buprenorphine ( BTDS ) .
	manualset3
119121	1	404732	5	NULL	NULL	NULL	NULL	PERSPECTIVE 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	PERSPECTIVE : This report demonstrates that the CHRONIC PAIN-CAT is feasible for administration in a clinic .
	manualset3
119122	2	404732	5	NULL	NULL	0	NULL	report 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	PERSPECTIVE : This report demonstrates that the CHRONIC PAIN-CAT is feasible for administration in a clinic .
	manualset3
119123	3	404732	5	NULL	NULL	0	NULL	CHRONIC PAIN-CAT 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	PERSPECTIVE : This report demonstrates that the CHRONIC PAIN-CAT is feasible for administration in a clinic .
	manualset3
119124	4	404732	5	NULL	NULL	0	NULL	administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	PERSPECTIVE : This report demonstrates that the CHRONIC PAIN-CAT is feasible for administration in a clinic .
	manualset3
119125	5	404732	5	NULL	NULL	0	NULL	clinic 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	PERSPECTIVE : This report demonstrates that the CHRONIC PAIN-CAT is feasible for administration in a clinic .
	manualset3
119126	1	404733	5	NULL	NULL	0	NULL	PET evaluation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	PET evaluation of soft-tissue masses with fluorine-18 fluoro-2-deoxy-D-glucose .
	manualset3
119127	2	404733	5	NULL	NULL	0	NULL	soft-tissue masses	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	PET evaluation of soft-tissue masses with fluorine-18 fluoro-2-deoxy-D-glucose .
	manualset3
119128	3	404733	5	NULL	NULL	0	NULL	fluorine-18 fluoro-2-deoxy-D-glucose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	PET evaluation of soft-tissue masses with fluorine-18 fluoro-2-deoxy-D-glucose .
	manualset3
119129	1	404734	5	NULL	NULL	0	NULL	PET 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	PET in cardiology : current status and clinical expectations .
	manualset3
119130	2	404734	5	NULL	NULL	0	NULL	cardiology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	PET in cardiology : current status and clinical expectations .
	manualset3
119131	3	404734	5	NULL	NULL	0	NULL	current status	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PET in cardiology : current status and clinical expectations .
	manualset3
119132	4	404734	5	NULL	NULL	0	NULL	clinical expectations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PET in cardiology : current status and clinical expectations .
	manualset3
119133	1	404735	5	NULL	NULL	0	NULL	PFAA concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PFAA concentrations and water discharge data were integrated into a mass balance assessment that shows that 30-60 % of PFAA loads can be attributed to diffuse inputs .
	manualset3
119134	2	404735	5	NULL	NULL	0	NULL	water discharge data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	PFAA concentrations and water discharge data were integrated into a mass balance assessment that shows that 30-60 % of PFAA loads can be attributed to diffuse inputs .
	manualset3
119135	3	404735	5	NULL	NULL	0	NULL	mass balance assessment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PFAA concentrations and water discharge data were integrated into a mass balance assessment that shows that 30-60 % of PFAA loads can be attributed to diffuse inputs .
	manualset3
119136	4	404735	5	NULL	NULL	0	NULL	 30-60 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	PFAA concentrations and water discharge data were integrated into a mass balance assessment that shows that 30-60 % of PFAA loads can be attributed to diffuse inputs .
	manualset3
119137	5	404735	5	NULL	NULL	0	NULL	PFAA loads 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	PFAA concentrations and water discharge data were integrated into a mass balance assessment that shows that 30-60 % of PFAA loads can be attributed to diffuse inputs .
	manualset3
119138	6	404735	5	NULL	NULL	0	NULL	diffuse inputs	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	PFAA concentrations and water discharge data were integrated into a mass balance assessment that shows that 30-60 % of PFAA loads can be attributed to diffuse inputs .
	manualset3
119139	1	404736	5	NULL	NULL	NULL	NULL	PFFA 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	PFFA has similarities to lichen planopilaris but is differentiated by a distinctive symmetrical fronto-temporal distribution and progressive course .
	manualset3
119140	2	404736	5	NULL	NULL	0	NULL	lichen planopilaris	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	PFFA has similarities to lichen planopilaris but is differentiated by a distinctive symmetrical fronto-temporal distribution and progressive course .
	manualset3
119141	3	404736	5	NULL	NULL	0	NULL	distinctive symmetrical fronto-temporal distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PFFA has similarities to lichen planopilaris but is differentiated by a distinctive symmetrical fronto-temporal distribution and progressive course .
	manualset3
119142	4	404736	5	NULL	NULL	0	NULL	progressive course	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PFFA has similarities to lichen planopilaris but is differentiated by a distinctive symmetrical fronto-temporal distribution and progressive course .
	manualset3
119143	1	404737	5	NULL	NULL	0	NULL	PFG-NMR-derived diffusion coefficients , D	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PFG-NMR-derived diffusion coefficients , D , provide a means for deriving the contribution of monomer and other oligomer states to this distribution .
	manualset3
119144	2	404737	5	NULL	NULL	0	NULL	contribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PFG-NMR-derived diffusion coefficients , D , provide a means for deriving the contribution of monomer and other oligomer states to this distribution .
	manualset3
119145	3	404737	5	NULL	NULL	0	NULL	monomer state	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	PFG-NMR-derived diffusion coefficients , D , provide a means for deriving the contribution of monomer and other oligomer states to this distribution .
	manualset3
119146	4	404737	5	NULL	NULL	0	NULL	oligomer state	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	PFG-NMR-derived diffusion coefficients , D , provide a means for deriving the contribution of monomer and other oligomer states to this distribution .
	manualset3
119147	5	404737	5	NULL	NULL	0	NULL	distribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PFG-NMR-derived diffusion coefficients , D , provide a means for deriving the contribution of monomer and other oligomer states to this distribution .
	manualset3
119148	1	404738	5	NULL	NULL	0	NULL	PGC-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PGC-1 promotes recovery after acute kidney injury during systemic inflammation in mice .
	manualset3
119149	2	404738	5	NULL	NULL	0	NULL	recovery 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	PGC-1 promotes recovery after acute kidney injury during systemic inflammation in mice .
	manualset3
119150	3	404738	5	NULL	NULL	0	NULL	acute kidney injury 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	PGC-1 promotes recovery after acute kidney injury during systemic inflammation in mice .
	manualset3
119151	4	404738	5	NULL	NULL	0	NULL	systemic inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	PGC-1 promotes recovery after acute kidney injury during systemic inflammation in mice .
	manualset3
119152	5	404738	5	NULL	NULL	0	NULL	mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	PGC-1 promotes recovery after acute kidney injury during systemic inflammation in mice .
	manualset3
119153	1	404739	5	NULL	NULL	0	NULL	PGC-1alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PGC-1alpha is not mandatory for exercise - and training-induced adaptive gene responses in mouse skeletal muscle .
	manualset3
119154	2	404739	5	NULL	NULL	0	NULL	exercise - induced adaptive gene responses	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PGC-1alpha is not mandatory for exercise - and training-induced adaptive gene responses in mouse skeletal muscle .
	manualset3
119155	3	404739	5	NULL	NULL	0	NULL	training-induced adaptive gene responses	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PGC-1alpha is not mandatory for exercise - and training-induced adaptive gene responses in mouse skeletal muscle .
	manualset3
119156	4	404739	5	NULL	NULL	0	NULL	mouse skeletal muscle 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	PGC-1alpha is not mandatory for exercise - and training-induced adaptive gene responses in mouse skeletal muscle .
	manualset3
119157	1	404740	5	NULL	NULL	0	NULL	PGE1 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	PGE1 desensitized the response to PGE2 and iloprost but not vice versa .
	manualset3
119158	2	404740	5	NULL	NULL	0	NULL	response 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PGE1 desensitized the response to PGE2 and iloprost but not vice versa .
	manualset3
119159	3	404740	5	NULL	NULL	0	NULL	PGE2 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	PGE1 desensitized the response to PGE2 and iloprost but not vice versa .
	manualset3
122298	4	404740	5	NULL	NULL	0	NULL	iloprost 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	PGE1 desensitized the response to PGE2 and iloprost but not vice versa .
	manualset3
119160	1	404741	5	NULL	NULL	0	NULL	PGE2	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	PGE2 inhibited 10 m U/ml vasopressin-induced osmotic water flow of the toad bladder at 2 X 10 ( -8 ) M. PGE2 suppressed vasopressin-mediated cyclic AMP accumulation in epithelial cells and also vasopressin-mediated adenylate cyclase activity in a crude homogenate of the cells .
	manualset3
119161	2	404741	5	NULL	NULL	0	NULL	10 m U/ml vasopressin-induced osmotic water flow 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	PGE2 inhibited 10 m U/ml vasopressin-induced osmotic water flow of the toad bladder at 2 X 10 ( -8 ) M. PGE2 suppressed vasopressin-mediated cyclic AMP accumulation in epithelial cells and also vasopressin-mediated adenylate cyclase activity in a crude homogenate of the cells .
	manualset3
119162	3	404741	5	NULL	NULL	0	NULL	toad bladder	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	PGE2 inhibited 10 m U/ml vasopressin-induced osmotic water flow of the toad bladder at 2 X 10 ( -8 ) M. PGE2 suppressed vasopressin-mediated cyclic AMP accumulation in epithelial cells and also vasopressin-mediated adenylate cyclase activity in a crude homogenate of the cells .
	manualset3
119163	4	404741	5	NULL	NULL	0	NULL	2 X 10 ( -8 ) M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	PGE2 inhibited 10 m U/ml vasopressin-induced osmotic water flow of the toad bladder at 2 X 10 ( -8 ) M. PGE2 suppressed vasopressin-mediated cyclic AMP accumulation in epithelial cells and also vasopressin-mediated adenylate cyclase activity in a crude homogenate of the cells .
	manualset3
119164	5	404741	5	NULL	NULL	0	NULL	PGE2 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	PGE2 inhibited 10 m U/ml vasopressin-induced osmotic water flow of the toad bladder at 2 X 10 ( -8 ) M. PGE2 suppressed vasopressin-mediated cyclic AMP accumulation in epithelial cells and also vasopressin-mediated adenylate cyclase activity in a crude homogenate of the cells .
	manualset3
119165	6	404741	5	NULL	NULL	0	NULL	vasopressin-mediated cyclic AMP accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PGE2 inhibited 10 m U/ml vasopressin-induced osmotic water flow of the toad bladder at 2 X 10 ( -8 ) M. PGE2 suppressed vasopressin-mediated cyclic AMP accumulation in epithelial cells and also vasopressin-mediated adenylate cyclase activity in a crude homogenate of the cells .
	manualset3
119166	7	404741	5	NULL	NULL	0	NULL	epithelial cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	PGE2 inhibited 10 m U/ml vasopressin-induced osmotic water flow of the toad bladder at 2 X 10 ( -8 ) M. PGE2 suppressed vasopressin-mediated cyclic AMP accumulation in epithelial cells and also vasopressin-mediated adenylate cyclase activity in a crude homogenate of the cells .
	manualset3
119170	8	404741	5	NULL	NULL	0	NULL	vasopressin-mediated adenylate cyclase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PGE2 inhibited 10 m U/ml vasopressin-induced osmotic water flow of the toad bladder at 2 X 10 ( -8 ) M. PGE2 suppressed vasopressin-mediated cyclic AMP accumulation in epithelial cells and also vasopressin-mediated adenylate cyclase activity in a crude homogenate of the cells .
	manualset3
119171	9	404741	5	NULL	NULL	0	NULL	crude homogenate	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	PGE2 inhibited 10 m U/ml vasopressin-induced osmotic water flow of the toad bladder at 2 X 10 ( -8 ) M. PGE2 suppressed vasopressin-mediated cyclic AMP accumulation in epithelial cells and also vasopressin-mediated adenylate cyclase activity in a crude homogenate of the cells .
	manualset3
119172	10	404741	5	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	PGE2 inhibited 10 m U/ml vasopressin-induced osmotic water flow of the toad bladder at 2 X 10 ( -8 ) M. PGE2 suppressed vasopressin-mediated cyclic AMP accumulation in epithelial cells and also vasopressin-mediated adenylate cyclase activity in a crude homogenate of the cells .
	manualset3
119173	1	404742	5	NULL	NULL	0	NULL	 follow-up measuring program	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A follow-up measuring program confirmed a clear improvement in reliability and a reduction in the imprecision , particularly for results from series to series .
	manualset3
119174	2	404742	5	NULL	NULL	0	NULL	clear improvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A follow-up measuring program confirmed a clear improvement in reliability and a reduction in the imprecision , particularly for results from series to series .
	manualset3
119175	3	404742	5	NULL	NULL	0	NULL	reliability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A follow-up measuring program confirmed a clear improvement in reliability and a reduction in the imprecision , particularly for results from series to series .
	manualset3
119176	4	404742	5	NULL	NULL	0	NULL	reduction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A follow-up measuring program confirmed a clear improvement in reliability and a reduction in the imprecision , particularly for results from series to series .
	manualset3
119180	5	404742	5	NULL	NULL	0	NULL	imprecision 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A follow-up measuring program confirmed a clear improvement in reliability and a reduction in the imprecision , particularly for results from series to series .
	manualset3
119204	6	404742	5	NULL	NULL	0	NULL	results 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A follow-up measuring program confirmed a clear improvement in reliability and a reduction in the imprecision , particularly for results from series to series .
	manualset3
119205	7	404742	5	NULL	NULL	0	NULL	series 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A follow-up measuring program confirmed a clear improvement in reliability and a reduction in the imprecision , particularly for results from series to series .
	manualset3
119206	8	404742	5	NULL	NULL	0	NULL	series 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A follow-up measuring program confirmed a clear improvement in reliability and a reduction in the imprecision , particularly for results from series to series .
	manualset3
119207	1	404743	5	NULL	NULL	NULL	NULL	PGF2 alpha	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	PGF2 alpha plasma level peaks in April , is low in summer , and progressively increases during autumn to peak again in December .
	manualset3
119208	2	404743	5	NULL	NULL	0	NULL	plasma level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PGF2 alpha plasma level peaks in April , is low in summer , and progressively increases during autumn to peak again in December .
	manualset3
119209	3	404743	5	NULL	NULL	0	NULL	April 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	PGF2 alpha plasma level peaks in April , is low in summer , and progressively increases during autumn to peak again in December .
	manualset3
119210	4	404743	5	NULL	NULL	NULL	NULL	summer 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	PGF2 alpha plasma level peaks in April , is low in summer , and progressively increases during autumn to peak again in December .
	manualset3
119211	5	404743	5	NULL	NULL	0	NULL	autumn 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	PGF2 alpha plasma level peaks in April , is low in summer , and progressively increases during autumn to peak again in December .
	manualset3
119212	6	404743	5	NULL	NULL	0	NULL	peak 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	PGF2 alpha plasma level peaks in April , is low in summer , and progressively increases during autumn to peak again in December .
	manualset3
119213	7	404743	5	NULL	NULL	0	NULL	December 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	PGF2 alpha plasma level peaks in April , is low in summer , and progressively increases during autumn to peak again in December .
	manualset3
119214	1	404744	5	NULL	NULL	0	NULL	PGLa	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PGLa , like magainin 2 , preferentially interacts with acidic lipids , forming an amphipathic helix .
	manualset3
119215	2	404744	5	NULL	NULL	0	NULL	magainin 2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PGLa , like magainin 2 , preferentially interacts with acidic lipids , forming an amphipathic helix .
	manualset3
119216	3	404744	5	NULL	NULL	0	NULL	acidic lipids	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	PGLa , like magainin 2 , preferentially interacts with acidic lipids , forming an amphipathic helix .
	manualset3
119217	4	404744	5	NULL	NULL	0	NULL	amphipathic helix	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	PGLa , like magainin 2 , preferentially interacts with acidic lipids , forming an amphipathic helix .
	manualset3
119218	1	404745	5	NULL	NULL	0	NULL	PGME 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	PGME was readily absorbed and metabolized to PG following oral gavage administration at 90 mg/kg .
	manualset3
119219	2	404745	5	NULL	NULL	0	NULL	PG 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	PGME was readily absorbed and metabolized to PG following oral gavage administration at 90 mg/kg .
	manualset3
119220	3	404745	5	NULL	NULL	0	NULL	oral gavage administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	PGME was readily absorbed and metabolized to PG following oral gavage administration at 90 mg/kg .
	manualset3
119221	4	404745	5	NULL	NULL	0	NULL	90 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	PGME was readily absorbed and metabolized to PG following oral gavage administration at 90 mg/kg .
	manualset3
119222	1	404746	5	NULL	NULL	NULL	NULL	PH 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	PH provides one example of the absolute need for workup of the metabolic causes of stone disease .
	manualset3
119223	2	404746	5	NULL	NULL	0	NULL	example 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	PH provides one example of the absolute need for workup of the metabolic causes of stone disease .
	manualset3
119224	3	404746	5	NULL	NULL	0	NULL	need 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PH provides one example of the absolute need for workup of the metabolic causes of stone disease .
	manualset3
119225	4	404746	5	NULL	NULL	0	NULL	workup 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PH provides one example of the absolute need for workup of the metabolic causes of stone disease .
	manualset3
119226	5	404746	5	NULL	NULL	0	NULL	metabolic causes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	PH provides one example of the absolute need for workup of the metabolic causes of stone disease .
	manualset3
119227	6	404746	5	NULL	NULL	0	NULL	stone disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	PH provides one example of the absolute need for workup of the metabolic causes of stone disease .
	manualset3
119228	1	404747	5	NULL	NULL	0	NULL	PHB 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	PHB was not detectable in any of the mutants containing the phbC mutation ; glycogen was not detectable in any of the mutants containing the glgA1 mutation .
	manualset3
119229	2	404747	5	NULL	NULL	0	NULL	mutants 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	PHB was not detectable in any of the mutants containing the phbC mutation ; glycogen was not detectable in any of the mutants containing the glgA1 mutation .
	manualset3
119230	3	404747	5	NULL	NULL	0	NULL	phbC mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PHB was not detectable in any of the mutants containing the phbC mutation ; glycogen was not detectable in any of the mutants containing the glgA1 mutation .
	manualset3
119231	4	404747	5	NULL	NULL	0	NULL	glycogen 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	PHB was not detectable in any of the mutants containing the phbC mutation ; glycogen was not detectable in any of the mutants containing the glgA1 mutation .
	manualset3
119232	5	404747	5	NULL	NULL	0	NULL	mutants 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	PHB was not detectable in any of the mutants containing the phbC mutation ; glycogen was not detectable in any of the mutants containing the glgA1 mutation .
	manualset3
119233	6	404747	5	NULL	NULL	0	NULL	glgA1 mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PHB was not detectable in any of the mutants containing the phbC mutation ; glycogen was not detectable in any of the mutants containing the glgA1 mutation .
	manualset3
119234	1	404748	5	NULL	NULL	0	NULL	PIA 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	PIA identified previously described null polymorphisms in glutathione-S-transferase T1 ( GSTT1 ) as the best predictor of colon cancer among the studied SNPs , and also identified novel polymorphisms in the inflammation and hormone metabolism pathways that singly or jointly predict cancer risk .
	manualset3
119235	2	404748	5	NULL	NULL	0	NULL	null polymorphisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PIA identified previously described null polymorphisms in glutathione-S-transferase T1 ( GSTT1 ) as the best predictor of colon cancer among the studied SNPs , and also identified novel polymorphisms in the inflammation and hormone metabolism pathways that singly or jointly predict cancer risk .
	manualset3
119236	3	404748	5	NULL	NULL	0	NULL	glutathione-S-transferase T1 ( GSTT1 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PIA identified previously described null polymorphisms in glutathione-S-transferase T1 ( GSTT1 ) as the best predictor of colon cancer among the studied SNPs , and also identified novel polymorphisms in the inflammation and hormone metabolism pathways that singly or jointly predict cancer risk .
	manualset3
119237	4	404748	5	NULL	NULL	0	NULL	best predictor 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	PIA identified previously described null polymorphisms in glutathione-S-transferase T1 ( GSTT1 ) as the best predictor of colon cancer among the studied SNPs , and also identified novel polymorphisms in the inflammation and hormone metabolism pathways that singly or jointly predict cancer risk .
	manualset3
119238	5	404748	5	NULL	NULL	0	NULL	colon cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	PIA identified previously described null polymorphisms in glutathione-S-transferase T1 ( GSTT1 ) as the best predictor of colon cancer among the studied SNPs , and also identified novel polymorphisms in the inflammation and hormone metabolism pathways that singly or jointly predict cancer risk .
	manualset3
119239	6	404748	5	NULL	NULL	0	NULL	SNPs 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	PIA identified previously described null polymorphisms in glutathione-S-transferase T1 ( GSTT1 ) as the best predictor of colon cancer among the studied SNPs , and also identified novel polymorphisms in the inflammation and hormone metabolism pathways that singly or jointly predict cancer risk .
	manualset3
119240	7	404748	5	NULL	NULL	0	NULL	novel polymorphisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PIA identified previously described null polymorphisms in glutathione-S-transferase T1 ( GSTT1 ) as the best predictor of colon cancer among the studied SNPs , and also identified novel polymorphisms in the inflammation and hormone metabolism pathways that singly or jointly predict cancer risk .
	manualset3
119241	8	404748	5	NULL	NULL	0	NULL	inflammation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PIA identified previously described null polymorphisms in glutathione-S-transferase T1 ( GSTT1 ) as the best predictor of colon cancer among the studied SNPs , and also identified novel polymorphisms in the inflammation and hormone metabolism pathways that singly or jointly predict cancer risk .
	manualset3
119242	9	404748	5	NULL	NULL	0	NULL	hormone metabolism pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PIA identified previously described null polymorphisms in glutathione-S-transferase T1 ( GSTT1 ) as the best predictor of colon cancer among the studied SNPs , and also identified novel polymorphisms in the inflammation and hormone metabolism pathways that singly or jointly predict cancer risk .
	manualset3
119243	10	404748	5	NULL	NULL	0	NULL	cancer risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	PIA identified previously described null polymorphisms in glutathione-S-transferase T1 ( GSTT1 ) as the best predictor of colon cancer among the studied SNPs , and also identified novel polymorphisms in the inflammation and hormone metabolism pathways that singly or jointly predict cancer risk .
	manualset3
119244	1	404749	5	NULL	NULL	0	NULL	PIG-induced pp59 ( Lyn ) kinase activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PIG-induced pp59 ( Lyn ) kinase activation and pp125 ( FAK ) tyrosine phosphorylation were impaired by the former and latter peptide , respectively .
	manualset3
119245	2	404749	5	NULL	NULL	0	NULL	pp125 ( FAK ) tyrosine phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PIG-induced pp59 ( Lyn ) kinase activation and pp125 ( FAK ) tyrosine phosphorylation were impaired by the former and latter peptide , respectively .
	manualset3
119246	3	404749	5	NULL	NULL	0	NULL	former peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	PIG-induced pp59 ( Lyn ) kinase activation and pp125 ( FAK ) tyrosine phosphorylation were impaired by the former and latter peptide , respectively .
	manualset3
119247	4	404749	5	NULL	NULL	0	NULL	latter peptide 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	PIG-induced pp59 ( Lyn ) kinase activation and pp125 ( FAK ) tyrosine phosphorylation were impaired by the former and latter peptide , respectively .
	manualset3
119248	1	404750	5	NULL	NULL	0	NULL	PIV3 infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	PIV3 infections were observed every year during the fall and winter , with peaks of infections in the spring in the years without PIV1 .
	manualset3
119249	2	404750	5	NULL	NULL	0	NULL	every year	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	PIV3 infections were observed every year during the fall and winter , with peaks of infections in the spring in the years without PIV1 .
	manualset3
119250	3	404750	5	NULL	NULL	0	NULL	fall 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	PIV3 infections were observed every year during the fall and winter , with peaks of infections in the spring in the years without PIV1 .
	manualset3
119251	4	404750	5	NULL	NULL	0	NULL	winter 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	PIV3 infections were observed every year during the fall and winter , with peaks of infections in the spring in the years without PIV1 .
	manualset3
119252	5	404750	5	NULL	NULL	0	NULL	peaks 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PIV3 infections were observed every year during the fall and winter , with peaks of infections in the spring in the years without PIV1 .
	manualset3
119253	6	404750	5	NULL	NULL	0	NULL	infections 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	PIV3 infections were observed every year during the fall and winter , with peaks of infections in the spring in the years without PIV1 .
	manualset3
119254	7	404750	5	NULL	NULL	0	NULL	spring 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	PIV3 infections were observed every year during the fall and winter , with peaks of infections in the spring in the years without PIV1 .
	manualset3
119255	8	404750	5	NULL	NULL	0	NULL	years 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	PIV3 infections were observed every year during the fall and winter , with peaks of infections in the spring in the years without PIV1 .
	manualset3
119256	9	404750	5	NULL	NULL	0	NULL	PIV1 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	PIV3 infections were observed every year during the fall and winter , with peaks of infections in the spring in the years without PIV1 .
	manualset3
119257	1	404751	5	NULL	NULL	0	NULL	formalism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A formalism is given in which the optical field generated by a near-field optical aperture is described as an analytic expansion over a complete set of optical modes .
	manualset3
119258	2	404751	5	NULL	NULL	0	NULL	optical field	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A formalism is given in which the optical field generated by a near-field optical aperture is described as an analytic expansion over a complete set of optical modes .
	manualset3
119259	3	404751	5	NULL	NULL	0	NULL	near-field optical aperture	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A formalism is given in which the optical field generated by a near-field optical aperture is described as an analytic expansion over a complete set of optical modes .
	manualset3
119260	4	404751	5	NULL	NULL	0	NULL	analytic expansion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A formalism is given in which the optical field generated by a near-field optical aperture is described as an analytic expansion over a complete set of optical modes .
	manualset3
119261	5	404751	5	NULL	NULL	0	NULL	complete set	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A formalism is given in which the optical field generated by a near-field optical aperture is described as an analytic expansion over a complete set of optical modes .
	manualset3
119262	6	404751	5	NULL	NULL	0	NULL	optical modes	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A formalism is given in which the optical field generated by a near-field optical aperture is described as an analytic expansion over a complete set of optical modes .
	manualset3
119263	1	404752	5	NULL	NULL	0	NULL	PIVET Medical Centre	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	PIVET Medical Centre has developed an empirical algorithm for the dose of FSH administration based upon day-2 FSH , antral follicle count , anti-Mllerian hormone , body mass index , age and smoking parameters in an attempt to reduce the incidence of ovarian hyperstimulation syndrome particularly in at-risk women with elevated antral follicle count and anti-Mllerian hormone .
	manualset3
119264	2	404752	5	NULL	NULL	0	NULL	empirical algorithm	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	PIVET Medical Centre has developed an empirical algorithm for the dose of FSH administration based upon day-2 FSH , antral follicle count , anti-Mllerian hormone , body mass index , age and smoking parameters in an attempt to reduce the incidence of ovarian hyperstimulation syndrome particularly in at-risk women with elevated antral follicle count and anti-Mllerian hormone .
	manualset3
119265	3	404752	5	NULL	NULL	0	NULL	dose 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PIVET Medical Centre has developed an empirical algorithm for the dose of FSH administration based upon day-2 FSH , antral follicle count , anti-Mllerian hormone , body mass index , age and smoking parameters in an attempt to reduce the incidence of ovarian hyperstimulation syndrome particularly in at-risk women with elevated antral follicle count and anti-Mllerian hormone .
	manualset3
119266	4	404752	5	NULL	NULL	0	NULL	FSH administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	PIVET Medical Centre has developed an empirical algorithm for the dose of FSH administration based upon day-2 FSH , antral follicle count , anti-Mllerian hormone , body mass index , age and smoking parameters in an attempt to reduce the incidence of ovarian hyperstimulation syndrome particularly in at-risk women with elevated antral follicle count and anti-Mllerian hormone .
	manualset3
119267	5	404752	5	NULL	NULL	NULL	NULL	FSH 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	PIVET Medical Centre has developed an empirical algorithm for the dose of FSH administration based upon day-2 FSH , antral follicle count , anti-Mllerian hormone , body mass index , age and smoking parameters in an attempt to reduce the incidence of ovarian hyperstimulation syndrome particularly in at-risk women with elevated antral follicle count and anti-Mllerian hormone .
	manualset3
119268	6	404752	5	NULL	NULL	0	NULL	antral follicle count	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PIVET Medical Centre has developed an empirical algorithm for the dose of FSH administration based upon day-2 FSH , antral follicle count , anti-Mllerian hormone , body mass index , age and smoking parameters in an attempt to reduce the incidence of ovarian hyperstimulation syndrome particularly in at-risk women with elevated antral follicle count and anti-Mllerian hormone .
	manualset3
119269	7	404752	5	NULL	NULL	0	NULL	anti-Mllerian hormone	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PIVET Medical Centre has developed an empirical algorithm for the dose of FSH administration based upon day-2 FSH , antral follicle count , anti-Mllerian hormone , body mass index , age and smoking parameters in an attempt to reduce the incidence of ovarian hyperstimulation syndrome particularly in at-risk women with elevated antral follicle count and anti-Mllerian hormone .
	manualset3
119270	8	404752	5	NULL	NULL	0	NULL	body mass index	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PIVET Medical Centre has developed an empirical algorithm for the dose of FSH administration based upon day-2 FSH , antral follicle count , anti-Mllerian hormone , body mass index , age and smoking parameters in an attempt to reduce the incidence of ovarian hyperstimulation syndrome particularly in at-risk women with elevated antral follicle count and anti-Mllerian hormone .
	manualset3
119271	9	404752	5	NULL	NULL	0	NULL	age 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	PIVET Medical Centre has developed an empirical algorithm for the dose of FSH administration based upon day-2 FSH , antral follicle count , anti-Mllerian hormone , body mass index , age and smoking parameters in an attempt to reduce the incidence of ovarian hyperstimulation syndrome particularly in at-risk women with elevated antral follicle count and anti-Mllerian hormone .
	manualset3
119272	10	404752	5	NULL	NULL	0	NULL	smoking parameters	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PIVET Medical Centre has developed an empirical algorithm for the dose of FSH administration based upon day-2 FSH , antral follicle count , anti-Mllerian hormone , body mass index , age and smoking parameters in an attempt to reduce the incidence of ovarian hyperstimulation syndrome particularly in at-risk women with elevated antral follicle count and anti-Mllerian hormone .
	manualset3
119273	11	404752	5	NULL	NULL	0	NULL	incidence 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PIVET Medical Centre has developed an empirical algorithm for the dose of FSH administration based upon day-2 FSH , antral follicle count , anti-Mllerian hormone , body mass index , age and smoking parameters in an attempt to reduce the incidence of ovarian hyperstimulation syndrome particularly in at-risk women with elevated antral follicle count and anti-Mllerian hormone .
	manualset3
119274	12	404752	5	NULL	NULL	0	NULL	ovarian hyperstimulation syndrome 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	PIVET Medical Centre has developed an empirical algorithm for the dose of FSH administration based upon day-2 FSH , antral follicle count , anti-Mllerian hormone , body mass index , age and smoking parameters in an attempt to reduce the incidence of ovarian hyperstimulation syndrome particularly in at-risk women with elevated antral follicle count and anti-Mllerian hormone .
	manualset3
119275	13	404752	5	NULL	NULL	0	NULL	at-risk women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	PIVET Medical Centre has developed an empirical algorithm for the dose of FSH administration based upon day-2 FSH , antral follicle count , anti-Mllerian hormone , body mass index , age and smoking parameters in an attempt to reduce the incidence of ovarian hyperstimulation syndrome particularly in at-risk women with elevated antral follicle count and anti-Mllerian hormone .
	manualset3
119276	14	404752	5	NULL	NULL	0	NULL	antral follicle count 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PIVET Medical Centre has developed an empirical algorithm for the dose of FSH administration based upon day-2 FSH , antral follicle count , anti-Mllerian hormone , body mass index , age and smoking parameters in an attempt to reduce the incidence of ovarian hyperstimulation syndrome particularly in at-risk women with elevated antral follicle count and anti-Mllerian hormone .
	manualset3
119277	15	404752	5	NULL	NULL	0	NULL	anti-Mllerian hormone	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PIVET Medical Centre has developed an empirical algorithm for the dose of FSH administration based upon day-2 FSH , antral follicle count , anti-Mllerian hormone , body mass index , age and smoking parameters in an attempt to reduce the incidence of ovarian hyperstimulation syndrome particularly in at-risk women with elevated antral follicle count and anti-Mllerian hormone .
	manualset3
119278	16	404752	5	NULL	NULL	0	NULL	day-2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	PIVET Medical Centre has developed an empirical algorithm for the dose of FSH administration based upon day-2 FSH , antral follicle count , anti-Mllerian hormone , body mass index , age and smoking parameters in an attempt to reduce the incidence of ovarian hyperstimulation syndrome particularly in at-risk women with elevated antral follicle count and anti-Mllerian hormone .
	manualset3
119279	1	404753	5	NULL	NULL	0	NULL	PLA2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PLA2 ( 15 , 600-62 , 500 U/l ) , the PLA2 activator melittin ( 0.5-20 mg/l ) and arachidonic acid ( 1 mmol/l ) all produced increases in ir-ACTH release from the cells , whilst platelet-activating factor ( PAF ) , prostaglandin F2 alpha ( PGF2 alpha ) , the prostacyclin analogs iloprost and BW245C , the thromboxane A2 ( TXA2 ) analog U46619 , and the leukotrienes LTB4 and LTC4 were ineffective in this respect .
	manualset3
119280	2	404753	5	NULL	NULL	0	NULL	 15 , 600-62 , 500 U/l 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	PLA2 ( 15 , 600-62 , 500 U/l ) , the PLA2 activator melittin ( 0.5-20 mg/l ) and arachidonic acid ( 1 mmol/l ) all produced increases in ir-ACTH release from the cells , whilst platelet-activating factor ( PAF ) , prostaglandin F2 alpha ( PGF2 alpha ) , the prostacyclin analogs iloprost and BW245C , the thromboxane A2 ( TXA2 ) analog U46619 , and the leukotrienes LTB4 and LTC4 were ineffective in this respect .
	manualset3
119281	3	404753	5	NULL	NULL	0	NULL	PLA2 activator melittin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	PLA2 ( 15 , 600-62 , 500 U/l ) , the PLA2 activator melittin ( 0.5-20 mg/l ) and arachidonic acid ( 1 mmol/l ) all produced increases in ir-ACTH release from the cells , whilst platelet-activating factor ( PAF ) , prostaglandin F2 alpha ( PGF2 alpha ) , the prostacyclin analogs iloprost and BW245C , the thromboxane A2 ( TXA2 ) analog U46619 , and the leukotrienes LTB4 and LTC4 were ineffective in this respect .
	manualset3
119282	4	404753	5	NULL	NULL	0	NULL	0.5-20 mg/l	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	PLA2 ( 15 , 600-62 , 500 U/l ) , the PLA2 activator melittin ( 0.5-20 mg/l ) and arachidonic acid ( 1 mmol/l ) all produced increases in ir-ACTH release from the cells , whilst platelet-activating factor ( PAF ) , prostaglandin F2 alpha ( PGF2 alpha ) , the prostacyclin analogs iloprost and BW245C , the thromboxane A2 ( TXA2 ) analog U46619 , and the leukotrienes LTB4 and LTC4 were ineffective in this respect .
	manualset3
119283	5	404753	5	NULL	NULL	0	NULL	arachidonic acid	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	PLA2 ( 15 , 600-62 , 500 U/l ) , the PLA2 activator melittin ( 0.5-20 mg/l ) and arachidonic acid ( 1 mmol/l ) all produced increases in ir-ACTH release from the cells , whilst platelet-activating factor ( PAF ) , prostaglandin F2 alpha ( PGF2 alpha ) , the prostacyclin analogs iloprost and BW245C , the thromboxane A2 ( TXA2 ) analog U46619 , and the leukotrienes LTB4 and LTC4 were ineffective in this respect .
	manualset3
119284	6	404753	5	NULL	NULL	0	NULL	 1 mmol/l 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	PLA2 ( 15 , 600-62 , 500 U/l ) , the PLA2 activator melittin ( 0.5-20 mg/l ) and arachidonic acid ( 1 mmol/l ) all produced increases in ir-ACTH release from the cells , whilst platelet-activating factor ( PAF ) , prostaglandin F2 alpha ( PGF2 alpha ) , the prostacyclin analogs iloprost and BW245C , the thromboxane A2 ( TXA2 ) analog U46619 , and the leukotrienes LTB4 and LTC4 were ineffective in this respect .
	manualset3
119285	7	404753	5	NULL	NULL	0	NULL	ir-ACTH release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PLA2 ( 15 , 600-62 , 500 U/l ) , the PLA2 activator melittin ( 0.5-20 mg/l ) and arachidonic acid ( 1 mmol/l ) all produced increases in ir-ACTH release from the cells , whilst platelet-activating factor ( PAF ) , prostaglandin F2 alpha ( PGF2 alpha ) , the prostacyclin analogs iloprost and BW245C , the thromboxane A2 ( TXA2 ) analog U46619 , and the leukotrienes LTB4 and LTC4 were ineffective in this respect .
	manualset3
119286	8	404753	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	PLA2 ( 15 , 600-62 , 500 U/l ) , the PLA2 activator melittin ( 0.5-20 mg/l ) and arachidonic acid ( 1 mmol/l ) all produced increases in ir-ACTH release from the cells , whilst platelet-activating factor ( PAF ) , prostaglandin F2 alpha ( PGF2 alpha ) , the prostacyclin analogs iloprost and BW245C , the thromboxane A2 ( TXA2 ) analog U46619 , and the leukotrienes LTB4 and LTC4 were ineffective in this respect .
	manualset3
119287	9	404753	5	NULL	NULL	0	NULL	platelet-activating factor ( PAF )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	PLA2 ( 15 , 600-62 , 500 U/l ) , the PLA2 activator melittin ( 0.5-20 mg/l ) and arachidonic acid ( 1 mmol/l ) all produced increases in ir-ACTH release from the cells , whilst platelet-activating factor ( PAF ) , prostaglandin F2 alpha ( PGF2 alpha ) , the prostacyclin analogs iloprost and BW245C , the thromboxane A2 ( TXA2 ) analog U46619 , and the leukotrienes LTB4 and LTC4 were ineffective in this respect .
	manualset3
119288	10	404753	5	NULL	NULL	0	NULL	prostaglandin F2 alpha ( PGF2 alpha )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	PLA2 ( 15 , 600-62 , 500 U/l ) , the PLA2 activator melittin ( 0.5-20 mg/l ) and arachidonic acid ( 1 mmol/l ) all produced increases in ir-ACTH release from the cells , whilst platelet-activating factor ( PAF ) , prostaglandin F2 alpha ( PGF2 alpha ) , the prostacyclin analogs iloprost and BW245C , the thromboxane A2 ( TXA2 ) analog U46619 , and the leukotrienes LTB4 and LTC4 were ineffective in this respect .
	manualset3
119289	11	404753	5	NULL	NULL	0	NULL	prostacyclin analog iloprost	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	PLA2 ( 15 , 600-62 , 500 U/l ) , the PLA2 activator melittin ( 0.5-20 mg/l ) and arachidonic acid ( 1 mmol/l ) all produced increases in ir-ACTH release from the cells , whilst platelet-activating factor ( PAF ) , prostaglandin F2 alpha ( PGF2 alpha ) , the prostacyclin analogs iloprost and BW245C , the thromboxane A2 ( TXA2 ) analog U46619 , and the leukotrienes LTB4 and LTC4 were ineffective in this respect .
	manualset3
119290	12	404753	5	NULL	NULL	0	NULL	prostacyclin analog BW245C 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	PLA2 ( 15 , 600-62 , 500 U/l ) , the PLA2 activator melittin ( 0.5-20 mg/l ) and arachidonic acid ( 1 mmol/l ) all produced increases in ir-ACTH release from the cells , whilst platelet-activating factor ( PAF ) , prostaglandin F2 alpha ( PGF2 alpha ) , the prostacyclin analogs iloprost and BW245C , the thromboxane A2 ( TXA2 ) analog U46619 , and the leukotrienes LTB4 and LTC4 were ineffective in this respect .
	manualset3
119291	13	404753	5	NULL	NULL	0	NULL	thromboxane A2 ( TXA2 ) analog U46619 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	PLA2 ( 15 , 600-62 , 500 U/l ) , the PLA2 activator melittin ( 0.5-20 mg/l ) and arachidonic acid ( 1 mmol/l ) all produced increases in ir-ACTH release from the cells , whilst platelet-activating factor ( PAF ) , prostaglandin F2 alpha ( PGF2 alpha ) , the prostacyclin analogs iloprost and BW245C , the thromboxane A2 ( TXA2 ) analog U46619 , and the leukotrienes LTB4 and LTC4 were ineffective in this respect .
	manualset3
119292	14	404753	5	NULL	NULL	0	NULL	leukotrienes LTB4 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	PLA2 ( 15 , 600-62 , 500 U/l ) , the PLA2 activator melittin ( 0.5-20 mg/l ) and arachidonic acid ( 1 mmol/l ) all produced increases in ir-ACTH release from the cells , whilst platelet-activating factor ( PAF ) , prostaglandin F2 alpha ( PGF2 alpha ) , the prostacyclin analogs iloprost and BW245C , the thromboxane A2 ( TXA2 ) analog U46619 , and the leukotrienes LTB4 and LTC4 were ineffective in this respect .
	manualset3
119293	15	404753	5	NULL	NULL	0	NULL	leukotrienes LTC4 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	PLA2 ( 15 , 600-62 , 500 U/l ) , the PLA2 activator melittin ( 0.5-20 mg/l ) and arachidonic acid ( 1 mmol/l ) all produced increases in ir-ACTH release from the cells , whilst platelet-activating factor ( PAF ) , prostaglandin F2 alpha ( PGF2 alpha ) , the prostacyclin analogs iloprost and BW245C , the thromboxane A2 ( TXA2 ) analog U46619 , and the leukotrienes LTB4 and LTC4 were ineffective in this respect .
	manualset3
119294	1	404754	5	NULL	NULL	0	NULL	PLACE 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	PLACE IN THERAPY : Agomelatine may represent a novel perspective in the treatment of acute depression .
	manualset3
119295	2	404754	5	NULL	NULL	0	NULL	THERAPY 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	PLACE IN THERAPY : Agomelatine may represent a novel perspective in the treatment of acute depression .
	manualset3
119296	3	404754	5	NULL	NULL	0	NULL	Agomelatine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	PLACE IN THERAPY : Agomelatine may represent a novel perspective in the treatment of acute depression .
	manualset3
119297	4	404754	5	NULL	NULL	0	NULL	perspective 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PLACE IN THERAPY : Agomelatine may represent a novel perspective in the treatment of acute depression .
	manualset3
119298	5	404754	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	PLACE IN THERAPY : Agomelatine may represent a novel perspective in the treatment of acute depression .
	manualset3
119299	6	404754	5	NULL	NULL	0	NULL	acute depression	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	PLACE IN THERAPY : Agomelatine may represent a novel perspective in the treatment of acute depression .
	manualset3
119300	1	404755	5	NULL	NULL	0	NULL	PM 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	PM and CO ( 2 ) were measured in thirty buses traveling between Taipei and Tainan .
	manualset3
119301	2	404755	5	NULL	NULL	0	NULL	CO ( 2 ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	PM and CO ( 2 ) were measured in thirty buses traveling between Taipei and Tainan .
	manualset3
119302	3	404755	5	NULL	NULL	0	NULL	thirty buses	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	PM and CO ( 2 ) were measured in thirty buses traveling between Taipei and Tainan .
	manualset3
119303	4	404755	5	NULL	NULL	0	NULL	Taipei 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	PM and CO ( 2 ) were measured in thirty buses traveling between Taipei and Tainan .
	manualset3
119304	5	404755	5	NULL	NULL	0	NULL	Tainan 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	PM and CO ( 2 ) were measured in thirty buses traveling between Taipei and Tainan .
	manualset3
119305	1	404756	5	NULL	NULL	0	NULL	PO	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PO then catalyzes the production of reactive compounds for microbe killing , wound healing , and melanin formation .
	manualset3
119306	2	404756	5	NULL	NULL	0	NULL	production 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PO then catalyzes the production of reactive compounds for microbe killing , wound healing , and melanin formation .
	manualset3
119307	3	404756	5	NULL	NULL	0	NULL	reactive compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	PO then catalyzes the production of reactive compounds for microbe killing , wound healing , and melanin formation .
	manualset3
119308	4	404756	5	NULL	NULL	NULL	NULL	microbe killing	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	PO then catalyzes the production of reactive compounds for microbe killing , wound healing , and melanin formation .
	manualset3
119309	5	404756	5	NULL	NULL	0	NULL	wound healing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PO then catalyzes the production of reactive compounds for microbe killing , wound healing , and melanin formation .
	manualset3
119310	6	404756	5	NULL	NULL	0	NULL	melanin formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PO then catalyzes the production of reactive compounds for microbe killing , wound healing , and melanin formation .
	manualset3
119311	1	404757	5	NULL	NULL	0	NULL	PO2-dependence	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PO2-dependence of phospholipase C in the cat carotid body .
	manualset3
119312	2	404757	5	NULL	NULL	0	NULL	phospholipase C 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PO2-dependence of phospholipase C in the cat carotid body .
	manualset3
119313	3	404757	5	NULL	NULL	0	NULL	cat carotid body 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	PO2-dependence of phospholipase C in the cat carotid body .
	manualset3
119314	1	404758	5	NULL	NULL	0	NULL	PP2A activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PP2A activation can be inhibited by mutation in the alpha 2 cytoplasmic domain and by a function-blocking anti-alpha 2 antibody .
	manualset3
119315	2	404758	5	NULL	NULL	0	NULL	mutation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PP2A activation can be inhibited by mutation in the alpha 2 cytoplasmic domain and by a function-blocking anti-alpha 2 antibody .
	manualset3
119316	3	404758	5	NULL	NULL	0	NULL	alpha 2 cytoplasmic domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	PP2A activation can be inhibited by mutation in the alpha 2 cytoplasmic domain and by a function-blocking anti-alpha 2 antibody .
	manualset3
119317	4	404758	5	NULL	NULL	0	NULL	function-blocking anti-alpha 2 antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PP2A activation can be inhibited by mutation in the alpha 2 cytoplasmic domain and by a function-blocking anti-alpha 2 antibody .
	manualset3
119318	1	404759	5	NULL	NULL	0	NULL	PPADS 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	PPADS at concentrations up to 100 microM had no effect on the EFS-induced response , indicating that this response is mediated through P2Y , but not P2X , receptor .
	manualset3
119319	2	404759	5	NULL	NULL	0	NULL	concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PPADS at concentrations up to 100 microM had no effect on the EFS-induced response , indicating that this response is mediated through P2Y , but not P2X , receptor .
	manualset3
119320	3	404759	5	NULL	NULL	0	NULL	100 microM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	PPADS at concentrations up to 100 microM had no effect on the EFS-induced response , indicating that this response is mediated through P2Y , but not P2X , receptor .
	manualset3
119321	4	404759	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PPADS at concentrations up to 100 microM had no effect on the EFS-induced response , indicating that this response is mediated through P2Y , but not P2X , receptor .
	manualset3
119322	5	404759	5	NULL	NULL	0	NULL	EFS-induced response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PPADS at concentrations up to 100 microM had no effect on the EFS-induced response , indicating that this response is mediated through P2Y , but not P2X , receptor .
	manualset3
119323	6	404759	5	NULL	NULL	0	NULL	response 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PPADS at concentrations up to 100 microM had no effect on the EFS-induced response , indicating that this response is mediated through P2Y , but not P2X , receptor .
	manualset3
119324	7	404759	5	NULL	NULL	0	NULL	P2Y 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PPADS at concentrations up to 100 microM had no effect on the EFS-induced response , indicating that this response is mediated through P2Y , but not P2X , receptor .
	manualset3
119325	8	404759	5	NULL	NULL	0	NULL	P2X , receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PPADS at concentrations up to 100 microM had no effect on the EFS-induced response , indicating that this response is mediated through P2Y , but not P2X , receptor .
	manualset3
119326	1	404760	5	NULL	NULL	0	NULL	PPAR-gamma receptor ligands	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	PPAR-gamma receptor ligands : novel therapy for pituitary adenomas .
	manualset3
119327	2	404760	5	NULL	NULL	0	NULL	novel therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	PPAR-gamma receptor ligands : novel therapy for pituitary adenomas .
	manualset3
119328	3	404760	5	NULL	NULL	0	NULL	pituitary adenomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	PPAR-gamma receptor ligands : novel therapy for pituitary adenomas .
	manualset3
119331	1	404761	5	NULL	NULL	0	NULL	PPARgamma mRNA expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PPARgamma mRNA expression was found in human peripheral blood T lymphocytes , raising the possibility of PPARgamma involvement in the regulation of T cell function .
	manualset3
119332	2	404761	5	NULL	NULL	0	NULL	human peripheral blood T lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	PPARgamma mRNA expression was found in human peripheral blood T lymphocytes , raising the possibility of PPARgamma involvement in the regulation of T cell function .
	manualset3
119333	3	404761	5	NULL	NULL	0	NULL	PPARgamma 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	PPARgamma mRNA expression was found in human peripheral blood T lymphocytes , raising the possibility of PPARgamma involvement in the regulation of T cell function .
	manualset3
119334	4	404761	5	NULL	NULL	0	NULL	regulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PPARgamma mRNA expression was found in human peripheral blood T lymphocytes , raising the possibility of PPARgamma involvement in the regulation of T cell function .
	manualset3
119335	5	404761	5	NULL	NULL	0	NULL	T cell function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PPARgamma mRNA expression was found in human peripheral blood T lymphocytes , raising the possibility of PPARgamma involvement in the regulation of T cell function .
	manualset3
119336	1	404762	5	NULL	NULL	0	NULL	 four-factor model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A four-factor model fit the data well , suggesting a distinction between clinical and personality disorders as well as a distinction between broad groups of internalizing and externalizing disorders .
	manualset3
119337	2	404762	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A four-factor model fit the data well , suggesting a distinction between clinical and personality disorders as well as a distinction between broad groups of internalizing and externalizing disorders .
	manualset3
119338	3	404762	5	NULL	NULL	0	NULL	distinction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A four-factor model fit the data well , suggesting a distinction between clinical and personality disorders as well as a distinction between broad groups of internalizing and externalizing disorders .
	manualset3
119339	4	404762	5	NULL	NULL	0	NULL	clinical disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A four-factor model fit the data well , suggesting a distinction between clinical and personality disorders as well as a distinction between broad groups of internalizing and externalizing disorders .
	manualset3
119340	5	404762	5	NULL	NULL	0	NULL	personality disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A four-factor model fit the data well , suggesting a distinction between clinical and personality disorders as well as a distinction between broad groups of internalizing and externalizing disorders .
	manualset3
119341	6	404762	5	NULL	NULL	0	NULL	broad groups 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A four-factor model fit the data well , suggesting a distinction between clinical and personality disorders as well as a distinction between broad groups of internalizing and externalizing disorders .
	manualset3
119342	7	404762	5	NULL	NULL	NULL	NULL	internalizing disorders	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A four-factor model fit the data well , suggesting a distinction between clinical and personality disorders as well as a distinction between broad groups of internalizing and externalizing disorders .
	manualset3
122299	8	404762	5	NULL	NULL	0	NULL	externalizing disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A four-factor model fit the data well , suggesting a distinction between clinical and personality disorders as well as a distinction between broad groups of internalizing and externalizing disorders .
	manualset3
119343	1	404763	5	NULL	NULL	0	NULL	PPCPs 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	PPCPs occur in low concentrations in the environment and are unlikely to elicit acute toxicity .
	manualset3
119344	2	404763	5	NULL	NULL	0	NULL	low concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PPCPs occur in low concentrations in the environment and are unlikely to elicit acute toxicity .
	manualset3
119345	3	404763	5	NULL	NULL	0	NULL	environment 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	PPCPs occur in low concentrations in the environment and are unlikely to elicit acute toxicity .
	manualset3
119346	4	404763	5	NULL	NULL	0	NULL	acute toxicity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PPCPs occur in low concentrations in the environment and are unlikely to elicit acute toxicity .
	manualset3
119347	1	404764	5	NULL	NULL	0	NULL	PPF 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PPF has also been used as a marker of MK maturation .
	manualset3
119348	2	404764	5	NULL	NULL	0	NULL	marker 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	PPF has also been used as a marker of MK maturation .
	manualset3
119349	3	404764	5	NULL	NULL	0	NULL	MK maturation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PPF has also been used as a marker of MK maturation .
	manualset3
119350	1	404765	5	NULL	NULL	0	NULL	PRCA 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	PRCA is thought to be an immunologically mediated disorder , but there is no uniformity in the setting of the management .
	manualset3
119351	2	404765	5	NULL	NULL	0	NULL	immunologically mediated disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	PRCA is thought to be an immunologically mediated disorder , but there is no uniformity in the setting of the management .
	manualset3
119352	3	404765	5	NULL	NULL	0	NULL	uniformity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PRCA is thought to be an immunologically mediated disorder , but there is no uniformity in the setting of the management .
	manualset3
119353	4	404765	5	NULL	NULL	0	NULL	management 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	PRCA is thought to be an immunologically mediated disorder , but there is no uniformity in the setting of the management .
	manualset3
119354	1	404766	5	NULL	NULL	0	NULL	PRL-IR 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PRL-IR was evident in the wall of vas efferens of tests and vas deferens .
	manualset3
119355	2	404766	5	NULL	NULL	0	NULL	wall of vas efferens 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	PRL-IR was evident in the wall of vas efferens of tests and vas deferens .
	manualset3
119356	3	404766	5	NULL	NULL	0	NULL	tests 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	PRL-IR was evident in the wall of vas efferens of tests and vas deferens .
	manualset3
119357	4	404766	5	NULL	NULL	0	NULL	vas deferens 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	PRL-IR was evident in the wall of vas efferens of tests and vas deferens .
	manualset3
119358	1	404767	5	NULL	NULL	0	NULL	PRL 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PRL , which is known to inhibit 20 alpha-SDH activity in regressing rat corpora lutea , suppressed the FSH-induced increase in enzyme activity in the granulosa cells .
	manualset3
119359	2	404767	5	NULL	NULL	0	NULL	20 alpha-SDH activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PRL , which is known to inhibit 20 alpha-SDH activity in regressing rat corpora lutea , suppressed the FSH-induced increase in enzyme activity in the granulosa cells .
	manualset3
119360	3	404767	5	NULL	NULL	0	NULL	regressing rat corpora lutea	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	PRL , which is known to inhibit 20 alpha-SDH activity in regressing rat corpora lutea , suppressed the FSH-induced increase in enzyme activity in the granulosa cells .
	manualset3
119361	4	404767	5	NULL	NULL	0	NULL	FSH-induced increase in enzyme activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PRL , which is known to inhibit 20 alpha-SDH activity in regressing rat corpora lutea , suppressed the FSH-induced increase in enzyme activity in the granulosa cells .
	manualset3
119362	5	404767	5	NULL	NULL	0	NULL	granulosa cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	PRL , which is known to inhibit 20 alpha-SDH activity in regressing rat corpora lutea , suppressed the FSH-induced increase in enzyme activity in the granulosa cells .
	manualset3
119363	1	404768	5	NULL	NULL	0	NULL	PSA 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PSA in the serum sample are allowed to react immunologically with the immobilized anti-tPSA and horseradish peroxidase ( HRP ) enzyme-labeled second antibodies specific to PSA .
	manualset3
119364	2	404768	5	NULL	NULL	0	NULL	serum sample	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	PSA in the serum sample are allowed to react immunologically with the immobilized anti-tPSA and horseradish peroxidase ( HRP ) enzyme-labeled second antibodies specific to PSA .
	manualset3
119365	3	404768	5	NULL	NULL	0	NULL	immobilized anti-tPSA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PSA in the serum sample are allowed to react immunologically with the immobilized anti-tPSA and horseradish peroxidase ( HRP ) enzyme-labeled second antibodies specific to PSA .
	manualset3
119366	4	404768	5	NULL	NULL	0	NULL	horseradish peroxidase ( HRP ) enzyme-labeled second antibodies specific to PSA	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	PSA in the serum sample are allowed to react immunologically with the immobilized anti-tPSA and horseradish peroxidase ( HRP ) enzyme-labeled second antibodies specific to PSA .
	manualset3
119367	1	404769	5	NULL	NULL	0	NULL	PSNs 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	PSNs will not become a national trend without a fight .
	manualset3
119368	2	404769	5	NULL	NULL	0	NULL	national trend	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PSNs will not become a national trend without a fight .
	manualset3
119369	3	404769	5	NULL	NULL	0	NULL	fight 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PSNs will not become a national trend without a fight .
	manualset3
119370	1	404770	5	NULL	NULL	0	NULL	fraction 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A fraction of these cells also expressed CD11c marker and appeared similar to inflammatory dendritic cells ( DCs ) .
	manualset3
119371	2	404770	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A fraction of these cells also expressed CD11c marker and appeared similar to inflammatory dendritic cells ( DCs ) .
	manualset3
119372	3	404770	5	NULL	NULL	0	NULL	 CD11c marker 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A fraction of these cells also expressed CD11c marker and appeared similar to inflammatory dendritic cells ( DCs ) .
	manualset3
119373	4	404770	5	NULL	NULL	0	NULL	inflammatory dendritic cells ( DCs ) 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A fraction of these cells also expressed CD11c marker and appeared similar to inflammatory dendritic cells ( DCs ) .
	manualset3
119374	1	404771	5	NULL	NULL	0	NULL	PSY-PR patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	PSY-PR patients were more frequently diagnosed as psychotic or affected by anxiety disorders .
	manualset3
119375	2	404771	5	NULL	NULL	0	NULL	 anxiety disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	PSY-PR patients were more frequently diagnosed as psychotic or affected by anxiety disorders .
	manualset3
119376	1	404772	5	NULL	NULL	0	NULL	PTH 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PTH ( 250 nM ) stimulated cytosolic PKA activity four - to fivefold within 30 s , and PKA activity was sustained for at least 5 min .
	manualset3
119377	2	404772	5	NULL	NULL	0	NULL	250 nM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	PTH ( 250 nM ) stimulated cytosolic PKA activity four - to fivefold within 30 s , and PKA activity was sustained for at least 5 min .
	manualset3
119378	3	404772	5	NULL	NULL	0	NULL	 cytosolic PKA activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PTH ( 250 nM ) stimulated cytosolic PKA activity four - to fivefold within 30 s , and PKA activity was sustained for at least 5 min .
	manualset3
119379	4	404772	5	NULL	NULL	0	NULL	 four - to fivefold 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	PTH ( 250 nM ) stimulated cytosolic PKA activity four - to fivefold within 30 s , and PKA activity was sustained for at least 5 min .
	manualset3
119380	5	404772	5	NULL	NULL	0	NULL	30 s	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	PTH ( 250 nM ) stimulated cytosolic PKA activity four - to fivefold within 30 s , and PKA activity was sustained for at least 5 min .
	manualset3
119381	6	404772	5	NULL	NULL	0	NULL	PKA activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PTH ( 250 nM ) stimulated cytosolic PKA activity four - to fivefold within 30 s , and PKA activity was sustained for at least 5 min .
	manualset3
119382	7	404772	5	NULL	NULL	0	NULL	5 min	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	PTH ( 250 nM ) stimulated cytosolic PKA activity four - to fivefold within 30 s , and PKA activity was sustained for at least 5 min .
	manualset3
119383	1	404773	5	NULL	NULL	0	NULL	PTH treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	PTH treatment induced substantial increases in bone mineral density ( BMD ) and trabecular bone volume in each mouse genotype .
	manualset3
119384	2	404773	5	NULL	NULL	0	NULL	bone mineral density ( BMD )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PTH treatment induced substantial increases in bone mineral density ( BMD ) and trabecular bone volume in each mouse genotype .
	manualset3
119385	3	404773	5	NULL	NULL	0	NULL	trabecular bone volume	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PTH treatment induced substantial increases in bone mineral density ( BMD ) and trabecular bone volume in each mouse genotype .
	manualset3
119386	4	404773	5	NULL	NULL	NULL	NULL	mouse genotype	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	PTH treatment induced substantial increases in bone mineral density ( BMD ) and trabecular bone volume in each mouse genotype .
	manualset3
119387	1	404774	5	NULL	NULL	0	NULL	PTSD 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	PTSD was assessed with regard to participants ' self-nominated worst event using the PTSD module of the SCID-I/NP ( First , Spitzer , Gibbon , & Williams , 1997 ) .
	manualset3
119388	2	404774	5	NULL	NULL	0	NULL	participant	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	PTSD was assessed with regard to participants ' self-nominated worst event using the PTSD module of the SCID-I/NP ( First , Spitzer , Gibbon , & Williams , 1997 ) .
	manualset3
119389	3	404774	5	NULL	NULL	0	NULL	self-nominated worst event	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PTSD was assessed with regard to participants ' self-nominated worst event using the PTSD module of the SCID-I/NP ( First , Spitzer , Gibbon , & Williams , 1997 ) .
	manualset3
119390	4	404774	5	NULL	NULL	0	NULL	PTSD module	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	PTSD was assessed with regard to participants ' self-nominated worst event using the PTSD module of the SCID-I/NP ( First , Spitzer , Gibbon , & Williams , 1997 ) .
	manualset3
119391	5	404774	5	NULL	NULL	NULL	NULL	SCID-I/NP	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	PTSD was assessed with regard to participants ' self-nominated worst event using the PTSD module of the SCID-I/NP ( First , Spitzer , Gibbon , & Williams , 1997 ) .
	manualset3
119392	6	404774	5	NULL	NULL	0	NULL	First , Spitzer , Gibbon , & Williams , 1997	Citation												NULL		0	NULL	NULL	NULL	NULL	NULL	PTSD was assessed with regard to participants ' self-nominated worst event using the PTSD module of the SCID-I/NP ( First , Spitzer , Gibbon , & Williams , 1997 ) .
	manualset3
119393	1	404775	5	NULL	NULL	0	NULL	PU .1 deletion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PU .1 deletion in granulocyte-macrophage progenitors , but not in common myeloid progenitors , resulted in excess granulocyte production ; this suggested specific roles of PU .1 at different stages of myeloid development .
	manualset3
119394	2	404775	5	NULL	NULL	0	NULL	granulocyte-macrophage progenitors	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	PU .1 deletion in granulocyte-macrophage progenitors , but not in common myeloid progenitors , resulted in excess granulocyte production ; this suggested specific roles of PU .1 at different stages of myeloid development .
	manualset3
119395	3	404775	5	NULL	NULL	0	NULL	myeloid progenitors	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	PU .1 deletion in granulocyte-macrophage progenitors , but not in common myeloid progenitors , resulted in excess granulocyte production ; this suggested specific roles of PU .1 at different stages of myeloid development .
	manualset3
119396	4	404775	5	NULL	NULL	0	NULL	excess granulocyte production	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	PU .1 deletion in granulocyte-macrophage progenitors , but not in common myeloid progenitors , resulted in excess granulocyte production ; this suggested specific roles of PU .1 at different stages of myeloid development .
	manualset3
119397	5	404775	5	NULL	NULL	0	NULL	specific roles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PU .1 deletion in granulocyte-macrophage progenitors , but not in common myeloid progenitors , resulted in excess granulocyte production ; this suggested specific roles of PU .1 at different stages of myeloid development .
	manualset3
119398	6	404775	5	NULL	NULL	0	NULL	PU .1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PU .1 deletion in granulocyte-macrophage progenitors , but not in common myeloid progenitors , resulted in excess granulocyte production ; this suggested specific roles of PU .1 at different stages of myeloid development .
	manualset3
119399	7	404775	5	NULL	NULL	0	NULL	different stages	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	PU .1 deletion in granulocyte-macrophage progenitors , but not in common myeloid progenitors , resulted in excess granulocyte production ; this suggested specific roles of PU .1 at different stages of myeloid development .
	manualset3
119400	8	404775	5	NULL	NULL	0	NULL	myeloid development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PU .1 deletion in granulocyte-macrophage progenitors , but not in common myeloid progenitors , resulted in excess granulocyte production ; this suggested specific roles of PU .1 at different stages of myeloid development .
	manualset3
119401	1	404776	5	NULL	NULL	0	NULL	PUFA feeding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PUFA feeding also increased the T3 receptor number without any significant change in its receptor affinity .
	manualset3
119402	2	404776	5	NULL	NULL	0	NULL	T3 receptor number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PUFA feeding also increased the T3 receptor number without any significant change in its receptor affinity .
	manualset3
119403	3	404776	5	NULL	NULL	0	NULL	significant change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PUFA feeding also increased the T3 receptor number without any significant change in its receptor affinity .
	manualset3
119404	4	404776	5	NULL	NULL	0	NULL	receptor affinity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PUFA feeding also increased the T3 receptor number without any significant change in its receptor affinity .
	manualset3
119405	1	404777	5	NULL	NULL	0	NULL	PURPOSE 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PURPOSE : Diagnosis Related Groups ( DRGs ) are widely used for a variety of purposes including quality improvement , hospital output measurement and funding .
	manualset3
119406	2	404777	5	NULL	NULL	0	NULL	Diagnosis Related Groups ( DRGs )	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	PURPOSE : Diagnosis Related Groups ( DRGs ) are widely used for a variety of purposes including quality improvement , hospital output measurement and funding .
	manualset3
119407	3	404777	5	NULL	NULL	0	NULL	purposes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PURPOSE : Diagnosis Related Groups ( DRGs ) are widely used for a variety of purposes including quality improvement , hospital output measurement and funding .
	manualset3
119408	4	404777	5	NULL	NULL	0	NULL	quality improvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PURPOSE : Diagnosis Related Groups ( DRGs ) are widely used for a variety of purposes including quality improvement , hospital output measurement and funding .
	manualset3
119409	5	404777	5	NULL	NULL	0	NULL	hospital output measurement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PURPOSE : Diagnosis Related Groups ( DRGs ) are widely used for a variety of purposes including quality improvement , hospital output measurement and funding .
	manualset3
119410	6	404777	5	NULL	NULL	0	NULL	funding 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PURPOSE : Diagnosis Related Groups ( DRGs ) are widely used for a variety of purposes including quality improvement , hospital output measurement and funding .
	manualset3
119411	1	404778	5	NULL	NULL	0	NULL	PURPOSE 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PURPOSE To develop a score predicting the risk of adverse events ( AEs ) in pediatric patients with cancer who experience fever and neutropenia ( FN ) and to evaluate its performance .
	manualset3
119425	2	404778	5	NULL	NULL	0	NULL	develop 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PURPOSE To develop a score predicting the risk of adverse events ( AEs ) in pediatric patients with cancer who experience fever and neutropenia ( FN ) and to evaluate its performance .
	manualset3
119426	3	404778	5	NULL	NULL	0	NULL	score 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PURPOSE To develop a score predicting the risk of adverse events ( AEs ) in pediatric patients with cancer who experience fever and neutropenia ( FN ) and to evaluate its performance .
	manualset3
119427	4	404778	5	NULL	NULL	0	NULL	risk 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PURPOSE To develop a score predicting the risk of adverse events ( AEs ) in pediatric patients with cancer who experience fever and neutropenia ( FN ) and to evaluate its performance .
	manualset3
119428	5	404778	5	NULL	NULL	0	NULL	adverse events ( AEs ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	PURPOSE To develop a score predicting the risk of adverse events ( AEs ) in pediatric patients with cancer who experience fever and neutropenia ( FN ) and to evaluate its performance .
	manualset3
119429	6	404778	5	NULL	NULL	0	NULL	pediatric patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	PURPOSE To develop a score predicting the risk of adverse events ( AEs ) in pediatric patients with cancer who experience fever and neutropenia ( FN ) and to evaluate its performance .
	manualset3
119430	7	404778	5	NULL	NULL	0	NULL	cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	PURPOSE To develop a score predicting the risk of adverse events ( AEs ) in pediatric patients with cancer who experience fever and neutropenia ( FN ) and to evaluate its performance .
	manualset3
119431	9	404778	5	NULL	NULL	NULL	NULL	fever 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	PURPOSE To develop a score predicting the risk of adverse events ( AEs ) in pediatric patients with cancer who experience fever and neutropenia ( FN ) and to evaluate its performance .
	manualset3
119432	10	404778	5	NULL	NULL	NULL	NULL	neutropenia ( FN )	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	PURPOSE To develop a score predicting the risk of adverse events ( AEs ) in pediatric patients with cancer who experience fever and neutropenia ( FN ) and to evaluate its performance .
	manualset3
119435	12	404778	5	NULL	NULL	0	NULL	performance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PURPOSE To develop a score predicting the risk of adverse events ( AEs ) in pediatric patients with cancer who experience fever and neutropenia ( FN ) and to evaluate its performance .
	manualset3
119436	1	404779	5	NULL	NULL	0	NULL	fragile secondary constriction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A fragile secondary constriction on chromosome 2 in a severely mentally retarded patient .
	manualset3
119437	2	404779	5	NULL	NULL	0	NULL	chromosome 2	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	A fragile secondary constriction on chromosome 2 in a severely mentally retarded patient .
	manualset3
119438	3	404779	5	NULL	NULL	0	NULL	severely mentally retarded patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A fragile secondary constriction on chromosome 2 in a severely mentally retarded patient .
	manualset3
119439	1	404780	5	NULL	NULL	0	NULL	PVR 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PVR decreased significantly to 212 + / - 99 dynes/sec/cm ( -5 ) ( p & lt ; 0.02 ) .
	manualset3
119440	2	404780	5	NULL	NULL	0	NULL	 212 + / - 99 dynes/sec/cm ( -5 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	PVR decreased significantly to 212 + / - 99 dynes/sec/cm ( -5 ) ( p & lt ; 0.02 ) .
	manualset3
119441	3	404780	5	NULL	NULL	0	NULL	 p & lt ; 0.02	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	PVR decreased significantly to 212 + / - 99 dynes/sec/cm ( -5 ) ( p & lt ; 0.02 ) .
	manualset3
119442	1	404781	5	NULL	NULL	0	NULL	PaCO2 removal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PaCO2 and CO2 removal for both coated and uncoated did not deteriorate significantly over the study .
	manualset3
119443	2	404781	5	NULL	NULL	0	NULL	CO2 removal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PaCO2 and CO2 removal for both coated and uncoated did not deteriorate significantly over the study .
	manualset3
119444	3	404781	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	PaCO2 and CO2 removal for both coated and uncoated did not deteriorate significantly over the study .
	manualset3
119445	1	404782	5	NULL	NULL	NULL	NULL	PaCO2 	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	PaCO2 rose from 44 to 70 ( fetus ) and 38 to 60 torr ( newborn ) with the addition of CO2 to room air .
	manualset3
119446	2	404782	5	NULL	NULL	0	NULL	44 to 70	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	PaCO2 rose from 44 to 70 ( fetus ) and 38 to 60 torr ( newborn ) with the addition of CO2 to room air .
	manualset3
119447	3	404782	5	NULL	NULL	0	NULL	fetus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	PaCO2 rose from 44 to 70 ( fetus ) and 38 to 60 torr ( newborn ) with the addition of CO2 to room air .
	manualset3
119448	4	404782	5	NULL	NULL	0	NULL	38 to 60 torr 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	PaCO2 rose from 44 to 70 ( fetus ) and 38 to 60 torr ( newborn ) with the addition of CO2 to room air .
	manualset3
119449	5	404782	5	NULL	NULL	0	NULL	newborn 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	PaCO2 rose from 44 to 70 ( fetus ) and 38 to 60 torr ( newborn ) with the addition of CO2 to room air .
	manualset3
119450	6	404782	5	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PaCO2 rose from 44 to 70 ( fetus ) and 38 to 60 torr ( newborn ) with the addition of CO2 to room air .
	manualset3
119451	7	404782	5	NULL	NULL	0	NULL	CO2 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	PaCO2 rose from 44 to 70 ( fetus ) and 38 to 60 torr ( newborn ) with the addition of CO2 to room air .
	manualset3
119452	8	404782	5	NULL	NULL	0	NULL	room air 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	PaCO2 rose from 44 to 70 ( fetus ) and 38 to 60 torr ( newborn ) with the addition of CO2 to room air .
	manualset3
119453	1	404783	5	NULL	NULL	0	NULL	PaO2	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	PaO2 in millimeters mercury : % FIO2 ratio and positive end-expiratory pressure were measured at 12-hour intervals , and hematocrit was measured at 6-hour intervals .
	manualset3
119454	2	404783	5	NULL	NULL	0	NULL	millimeters mercury	Unit												NULL		0	NULL	NULL	NULL	NULL	NULL	PaO2 in millimeters mercury : % FIO2 ratio and positive end-expiratory pressure were measured at 12-hour intervals , and hematocrit was measured at 6-hour intervals .
	manualset3
119455	3	404783	5	NULL	NULL	0	NULL	% FIO2 ratio 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PaO2 in millimeters mercury : % FIO2 ratio and positive end-expiratory pressure were measured at 12-hour intervals , and hematocrit was measured at 6-hour intervals .
	manualset3
119456	4	404783	5	NULL	NULL	0	NULL	positive end-expiratory pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PaO2 in millimeters mercury : % FIO2 ratio and positive end-expiratory pressure were measured at 12-hour intervals , and hematocrit was measured at 6-hour intervals .
	manualset3
119457	5	404783	5	NULL	NULL	0	NULL	12-hour intervals	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	PaO2 in millimeters mercury : % FIO2 ratio and positive end-expiratory pressure were measured at 12-hour intervals , and hematocrit was measured at 6-hour intervals .
	manualset3
119458	6	404783	5	NULL	NULL	0	NULL	hematocrit 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PaO2 in millimeters mercury : % FIO2 ratio and positive end-expiratory pressure were measured at 12-hour intervals , and hematocrit was measured at 6-hour intervals .
	manualset3
119459	7	404783	5	NULL	NULL	0	NULL	6-hour intervals	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	PaO2 in millimeters mercury : % FIO2 ratio and positive end-expiratory pressure were measured at 12-hour intervals , and hematocrit was measured at 6-hour intervals .
	manualset3
119460	1	404784	5	NULL	NULL	0	NULL	Paeciloxanthone 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Paeciloxanthone ( 1 ) , a new xanthone , and the known compounds emodin ( 2 ) and chrysophanol ( 3 ) , were isolated from the extract .
	manualset3
119461	2	404784	5	NULL	NULL	0	NULL	xanthone 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Paeciloxanthone ( 1 ) , a new xanthone , and the known compounds emodin ( 2 ) and chrysophanol ( 3 ) , were isolated from the extract .
	manualset3
119462	3	404784	5	NULL	NULL	0	NULL	emodin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Paeciloxanthone ( 1 ) , a new xanthone , and the known compounds emodin ( 2 ) and chrysophanol ( 3 ) , were isolated from the extract .
	manualset3
119463	4	404784	5	NULL	NULL	0	NULL	chrysophanol 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Paeciloxanthone ( 1 ) , a new xanthone , and the known compounds emodin ( 2 ) and chrysophanol ( 3 ) , were isolated from the extract .
	manualset3
119464	5	404784	5	NULL	NULL	0	NULL	extract 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Paeciloxanthone ( 1 ) , a new xanthone , and the known compounds emodin ( 2 ) and chrysophanol ( 3 ) , were isolated from the extract .
	manualset3
119465	1	404785	5	NULL	NULL	0	NULL	Paget 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Paget 's disease of the vulva is a rare entity ; since it may show the same clinical symptoms as benign chronic vulvitis , it may result in a delayed diagnosis .
	manualset3
119466	2	404785	5	NULL	NULL	0	NULL	vulva 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Paget 's disease of the vulva is a rare entity ; since it may show the same clinical symptoms as benign chronic vulvitis , it may result in a delayed diagnosis .
	manualset3
119467	3	404785	5	NULL	NULL	0	NULL	rare entity 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Paget 's disease of the vulva is a rare entity ; since it may show the same clinical symptoms as benign chronic vulvitis , it may result in a delayed diagnosis .
	manualset3
119468	4	404785	5	NULL	NULL	0	NULL	clinical symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Paget 's disease of the vulva is a rare entity ; since it may show the same clinical symptoms as benign chronic vulvitis , it may result in a delayed diagnosis .
	manualset3
119469	5	404785	5	NULL	NULL	0	NULL	benign chronic vulvitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Paget 's disease of the vulva is a rare entity ; since it may show the same clinical symptoms as benign chronic vulvitis , it may result in a delayed diagnosis .
	manualset3
119470	6	404785	5	NULL	NULL	0	NULL	delayed diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Paget 's disease of the vulva is a rare entity ; since it may show the same clinical symptoms as benign chronic vulvitis , it may result in a delayed diagnosis .
	manualset3
119471	1	404786	5	NULL	NULL	NULL	NULL	PaiA 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	PaiA shares recognizable sequence homology with N-acetyltransferases , including those that can acetylate spermidine/spermine substrates .
	manualset3
119472	2	404786	5	NULL	NULL	0	NULL	recognizable sequence homology	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PaiA shares recognizable sequence homology with N-acetyltransferases , including those that can acetylate spermidine/spermine substrates .
	manualset3
119473	3	404786	5	NULL	NULL	0	NULL	N-acetyltransferases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	PaiA shares recognizable sequence homology with N-acetyltransferases , including those that can acetylate spermidine/spermine substrates .
	manualset3
119474	4	404786	5	NULL	NULL	0	NULL	acetylate 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PaiA shares recognizable sequence homology with N-acetyltransferases , including those that can acetylate spermidine/spermine substrates .
	manualset3
119475	5	404786	5	NULL	NULL	0	NULL	spermidine/spermine substrates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	PaiA shares recognizable sequence homology with N-acetyltransferases , including those that can acetylate spermidine/spermine substrates .
	manualset3
119476	1	404787	5	NULL	NULL	0	NULL	Pain 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pain and thermal sensation in the cold : the effect of interval versus continuous exercise .
	manualset3
119477	2	404787	5	NULL	NULL	0	NULL	thermal sensation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pain and thermal sensation in the cold : the effect of interval versus continuous exercise .
	manualset3
119478	3	404787	5	NULL	NULL	0	NULL	cold 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Pain and thermal sensation in the cold : the effect of interval versus continuous exercise .
	manualset3
119479	4	404787	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pain and thermal sensation in the cold : the effect of interval versus continuous exercise .
	manualset3
119480	5	404787	5	NULL	NULL	0	NULL	interval exercise 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pain and thermal sensation in the cold : the effect of interval versus continuous exercise .
	manualset3
119481	6	404787	5	NULL	NULL	0	NULL	continuous exercise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pain and thermal sensation in the cold : the effect of interval versus continuous exercise .
	manualset3
119482	1	404788	5	NULL	NULL	NULL	NULL	framework 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A framework for making the necessary changes to the hospital disaster plan is presented .
	manualset3
119483	2	404788	5	NULL	NULL	0	NULL	changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A framework for making the necessary changes to the hospital disaster plan is presented .
	manualset3
119484	3	404788	5	NULL	NULL	0	NULL	hospital disaster plan	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A framework for making the necessary changes to the hospital disaster plan is presented .
	manualset3
119485	1	404789	5	NULL	NULL	0	NULL	Pain 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pain is the most commonly presenting symptom of acute aortic syndrome and should prompt immediate attention including diagnostic imaging modalities ( such as multislice computed tomography , transesophageal ultrasound , or magnetic resonance imaging ) .
	manualset3
119486	2	404789	5	NULL	NULL	0	NULL	most commonly presenting symptom	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pain is the most commonly presenting symptom of acute aortic syndrome and should prompt immediate attention including diagnostic imaging modalities ( such as multislice computed tomography , transesophageal ultrasound , or magnetic resonance imaging ) .
	manualset3
119487	3	404789	5	NULL	NULL	0	NULL	acute aortic syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pain is the most commonly presenting symptom of acute aortic syndrome and should prompt immediate attention including diagnostic imaging modalities ( such as multislice computed tomography , transesophageal ultrasound , or magnetic resonance imaging ) .
	manualset3
119488	4	404789	5	NULL	NULL	0	NULL	attention 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pain is the most commonly presenting symptom of acute aortic syndrome and should prompt immediate attention including diagnostic imaging modalities ( such as multislice computed tomography , transesophageal ultrasound , or magnetic resonance imaging ) .
	manualset3
119489	5	404789	5	NULL	NULL	0	NULL	diagnostic imaging modalities 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pain is the most commonly presenting symptom of acute aortic syndrome and should prompt immediate attention including diagnostic imaging modalities ( such as multislice computed tomography , transesophageal ultrasound , or magnetic resonance imaging ) .
	manualset3
119490	6	404789	5	NULL	NULL	0	NULL	multislice computed tomography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pain is the most commonly presenting symptom of acute aortic syndrome and should prompt immediate attention including diagnostic imaging modalities ( such as multislice computed tomography , transesophageal ultrasound , or magnetic resonance imaging ) .
	manualset3
119491	7	404789	5	NULL	NULL	0	NULL	transesophageal ultrasound	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pain is the most commonly presenting symptom of acute aortic syndrome and should prompt immediate attention including diagnostic imaging modalities ( such as multislice computed tomography , transesophageal ultrasound , or magnetic resonance imaging ) .
	manualset3
119492	8	404789	5	NULL	NULL	NULL	NULL	magnetic resonance imaging	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pain is the most commonly presenting symptom of acute aortic syndrome and should prompt immediate attention including diagnostic imaging modalities ( such as multislice computed tomography , transesophageal ultrasound , or magnetic resonance imaging ) .
	manualset3
119493	1	404790	5	NULL	NULL	0	NULL	Pain levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pain levels were found to be reduced after the relaxation exercises compared with the levels before the relaxation exercises ( z = -5.497 ; p & lt ; .001 ) .
	manualset3
119494	2	404790	5	NULL	NULL	0	NULL	relaxation exercises 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pain levels were found to be reduced after the relaxation exercises compared with the levels before the relaxation exercises ( z = -5.497 ; p & lt ; .001 ) .
	manualset3
119495	3	404790	5	NULL	NULL	0	NULL	levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pain levels were found to be reduced after the relaxation exercises compared with the levels before the relaxation exercises ( z = -5.497 ; p & lt ; .001 ) .
	manualset3
119496	4	404790	5	NULL	NULL	0	NULL	relaxation exercises	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pain levels were found to be reduced after the relaxation exercises compared with the levels before the relaxation exercises ( z = -5.497 ; p & lt ; .001 ) .
	manualset3
119497	5	404790	5	NULL	NULL	0	NULL	z = -5.497 ; p & lt ; .001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pain levels were found to be reduced after the relaxation exercises compared with the levels before the relaxation exercises ( z = -5.497 ; p & lt ; .001 ) .
	manualset3
119498	1	404791	5	NULL	NULL	0	NULL	Pain and depression scores	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pain and depression scores were significantly lower after the exercise program in the exercise group than in the control group .
	manualset3
119499	2	404791	5	NULL	NULL	0	NULL	exercise program	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pain and depression scores were significantly lower after the exercise program in the exercise group than in the control group .
	manualset3
119500	3	404791	5	NULL	NULL	0	NULL	exercise group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Pain and depression scores were significantly lower after the exercise program in the exercise group than in the control group .
	manualset3
119501	4	404791	5	NULL	NULL	0	NULL	control group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Pain and depression scores were significantly lower after the exercise program in the exercise group than in the control group .
	manualset3
119502	1	404792	5	NULL	NULL	NULL	NULL	Pain tolerance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pain tolerance and its predictability through ratings and psychological tests .
	manualset3
119503	2	404792	5	NULL	NULL	0	NULL	predictability 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pain tolerance and its predictability through ratings and psychological tests .
	manualset3
119504	3	404792	5	NULL	NULL	NULL	NULL	ratings 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pain tolerance and its predictability through ratings and psychological tests .
	manualset3
119505	4	404792	5	NULL	NULL	0	NULL	psychological tests	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pain tolerance and its predictability through ratings and psychological tests .
	manualset3
119506	1	404793	5	NULL	NULL	0	NULL	CLINICAL ASPECTS 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( CLINICAL AND HORMONAL ASPECTS OF ADRENAL CORTEX HYPERFUNCTION ) .
	manualset3
119507	2	404793	5	NULL	NULL	0	NULL	HORMONAL ASPECTS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( CLINICAL AND HORMONAL ASPECTS OF ADRENAL CORTEX HYPERFUNCTION ) .
	manualset3
119508	3	404793	5	NULL	NULL	0	NULL	ADRENAL CORTEX HYPERFUNCTION	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( CLINICAL AND HORMONAL ASPECTS OF ADRENAL CORTEX HYPERFUNCTION ) .
	manualset3
119509	1	404794	5	NULL	NULL	0	NULL	framework 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A framework for the mechanism by which elemental diet works , centering around the importance of the integrity of the intestinal barrier function , is proposed , and also appears to provide a logical explanation for some relapses of the disease .
	manualset3
119510	2	404794	5	NULL	NULL	0	NULL	mechanism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A framework for the mechanism by which elemental diet works , centering around the importance of the integrity of the intestinal barrier function , is proposed , and also appears to provide a logical explanation for some relapses of the disease .
	manualset3
119511	3	404794	5	NULL	NULL	0	NULL	elemental diet 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A framework for the mechanism by which elemental diet works , centering around the importance of the integrity of the intestinal barrier function , is proposed , and also appears to provide a logical explanation for some relapses of the disease .
	manualset3
119512	4	404794	5	NULL	NULL	0	NULL	importance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A framework for the mechanism by which elemental diet works , centering around the importance of the integrity of the intestinal barrier function , is proposed , and also appears to provide a logical explanation for some relapses of the disease .
	manualset3
119513	5	404794	5	NULL	NULL	0	NULL	integrity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A framework for the mechanism by which elemental diet works , centering around the importance of the integrity of the intestinal barrier function , is proposed , and also appears to provide a logical explanation for some relapses of the disease .
	manualset3
119514	6	404794	5	NULL	NULL	0	NULL	intestinal barrier function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A framework for the mechanism by which elemental diet works , centering around the importance of the integrity of the intestinal barrier function , is proposed , and also appears to provide a logical explanation for some relapses of the disease .
	manualset3
119515	7	404794	5	NULL	NULL	0	NULL	logical explanation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A framework for the mechanism by which elemental diet works , centering around the importance of the integrity of the intestinal barrier function , is proposed , and also appears to provide a logical explanation for some relapses of the disease .
	manualset3
119516	8	404794	5	NULL	NULL	0	NULL	relapses 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A framework for the mechanism by which elemental diet works , centering around the importance of the integrity of the intestinal barrier function , is proposed , and also appears to provide a logical explanation for some relapses of the disease .
	manualset3
119517	9	404794	5	NULL	NULL	0	NULL	disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A framework for the mechanism by which elemental diet works , centering around the importance of the integrity of the intestinal barrier function , is proposed , and also appears to provide a logical explanation for some relapses of the disease .
	manualset3
119518	1	404795	5	NULL	NULL	0	NULL	Paired cat corneas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Paired cat corneas , in either Optisol only or Optisol with growth factor ( s ) , were analyzed using ex vivo 31P nuclear magnetic resonance , after storage for 1 week at 4 degrees C. Lysosomal enzyme release into the media at the end of the storage period also was measured fluorometrically .
	manualset3
119519	2	404795	5	NULL	NULL	0	NULL	Optisol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Paired cat corneas , in either Optisol only or Optisol with growth factor ( s ) , were analyzed using ex vivo 31P nuclear magnetic resonance , after storage for 1 week at 4 degrees C. Lysosomal enzyme release into the media at the end of the storage period also was measured fluorometrically .
	manualset3
119520	3	404795	5	NULL	NULL	0	NULL	Optisol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Paired cat corneas , in either Optisol only or Optisol with growth factor ( s ) , were analyzed using ex vivo 31P nuclear magnetic resonance , after storage for 1 week at 4 degrees C. Lysosomal enzyme release into the media at the end of the storage period also was measured fluorometrically .
	manualset3
119521	4	404795	5	NULL	NULL	0	NULL	growth factor ( s )	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Paired cat corneas , in either Optisol only or Optisol with growth factor ( s ) , were analyzed using ex vivo 31P nuclear magnetic resonance , after storage for 1 week at 4 degrees C. Lysosomal enzyme release into the media at the end of the storage period also was measured fluorometrically .
	manualset3
119522	5	404795	5	NULL	NULL	0	NULL	ex vivo 31P nuclear magnetic resonance	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Paired cat corneas , in either Optisol only or Optisol with growth factor ( s ) , were analyzed using ex vivo 31P nuclear magnetic resonance , after storage for 1 week at 4 degrees C. Lysosomal enzyme release into the media at the end of the storage period also was measured fluorometrically .
	manualset3
119523	6	404795	5	NULL	NULL	0	NULL	storage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Paired cat corneas , in either Optisol only or Optisol with growth factor ( s ) , were analyzed using ex vivo 31P nuclear magnetic resonance , after storage for 1 week at 4 degrees C. Lysosomal enzyme release into the media at the end of the storage period also was measured fluorometrically .
	manualset3
119524	7	404795	5	NULL	NULL	0	NULL	 1 week 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Paired cat corneas , in either Optisol only or Optisol with growth factor ( s ) , were analyzed using ex vivo 31P nuclear magnetic resonance , after storage for 1 week at 4 degrees C. Lysosomal enzyme release into the media at the end of the storage period also was measured fluorometrically .
	manualset3
119525	8	404795	5	NULL	NULL	0	NULL	4 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Paired cat corneas , in either Optisol only or Optisol with growth factor ( s ) , were analyzed using ex vivo 31P nuclear magnetic resonance , after storage for 1 week at 4 degrees C. Lysosomal enzyme release into the media at the end of the storage period also was measured fluorometrically .
	manualset3
119526	9	404795	5	NULL	NULL	0	NULL	Lysosomal enzyme release 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Paired cat corneas , in either Optisol only or Optisol with growth factor ( s ) , were analyzed using ex vivo 31P nuclear magnetic resonance , after storage for 1 week at 4 degrees C. Lysosomal enzyme release into the media at the end of the storage period also was measured fluorometrically .
	manualset3
119527	10	404795	5	NULL	NULL	0	NULL	media 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Paired cat corneas , in either Optisol only or Optisol with growth factor ( s ) , were analyzed using ex vivo 31P nuclear magnetic resonance , after storage for 1 week at 4 degrees C. Lysosomal enzyme release into the media at the end of the storage period also was measured fluorometrically .
	manualset3
119528	11	404795	5	NULL	NULL	0	NULL	storage period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Paired cat corneas , in either Optisol only or Optisol with growth factor ( s ) , were analyzed using ex vivo 31P nuclear magnetic resonance , after storage for 1 week at 4 degrees C. Lysosomal enzyme release into the media at the end of the storage period also was measured fluorometrically .
	manualset3
119529	1	404796	5	NULL	NULL	0	NULL	AFLP distances 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pairwise AFLP distances that distinguish known clones from nonclones have been used to identify a threshold genetic dissimilarity distance below which samples are considered to represent a single clone .
	manualset3
119530	2	404796	5	NULL	NULL	0	NULL	known clones	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Pairwise AFLP distances that distinguish known clones from nonclones have been used to identify a threshold genetic dissimilarity distance below which samples are considered to represent a single clone .
	manualset3
119531	3	404796	5	NULL	NULL	0	NULL	nonclones 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Pairwise AFLP distances that distinguish known clones from nonclones have been used to identify a threshold genetic dissimilarity distance below which samples are considered to represent a single clone .
	manualset3
119532	4	404796	5	NULL	NULL	0	NULL	threshold genetic dissimilarity distance 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pairwise AFLP distances that distinguish known clones from nonclones have been used to identify a threshold genetic dissimilarity distance below which samples are considered to represent a single clone .
	manualset3
119533	5	404796	5	NULL	NULL	NULL	NULL	samples 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pairwise AFLP distances that distinguish known clones from nonclones have been used to identify a threshold genetic dissimilarity distance below which samples are considered to represent a single clone .
	manualset3
119534	6	404796	5	NULL	NULL	0	NULL	single clone 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Pairwise AFLP distances that distinguish known clones from nonclones have been used to identify a threshold genetic dissimilarity distance below which samples are considered to represent a single clone .
	manualset3
119535	1	404797	5	NULL	NULL	0	NULL	Pallister-Killian syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pallister-Killian syndrome : meiosis II non-disjunction may be the first step in the formation of isochromosome 12p .
	manualset3
119536	2	404797	5	NULL	NULL	0	NULL	meiosis II non-disjunction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pallister-Killian syndrome : meiosis II non-disjunction may be the first step in the formation of isochromosome 12p .
	manualset3
119537	3	404797	5	NULL	NULL	0	NULL	first step	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pallister-Killian syndrome : meiosis II non-disjunction may be the first step in the formation of isochromosome 12p .
	manualset3
119538	4	404797	5	NULL	NULL	0	NULL	formation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pallister-Killian syndrome : meiosis II non-disjunction may be the first step in the formation of isochromosome 12p .
	manualset3
119539	5	404797	5	NULL	NULL	0	NULL	isochromosome 12p	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Pallister-Killian syndrome : meiosis II non-disjunction may be the first step in the formation of isochromosome 12p .
	manualset3
119540	1	404798	5	NULL	NULL	0	NULL	Palmar keratin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Palmar and plantar keratin contained additional polypeptide chains and had a different size distribution compared with forearm and scalp keratin components .
	manualset3
119541	2	404798	5	NULL	NULL	0	NULL	plantar keratin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Palmar and plantar keratin contained additional polypeptide chains and had a different size distribution compared with forearm and scalp keratin components .
	manualset3
119542	3	404798	5	NULL	NULL	0	NULL	polypeptide chains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Palmar and plantar keratin contained additional polypeptide chains and had a different size distribution compared with forearm and scalp keratin components .
	manualset3
119543	4	404798	5	NULL	NULL	0	NULL	different size distribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Palmar and plantar keratin contained additional polypeptide chains and had a different size distribution compared with forearm and scalp keratin components .
	manualset3
119544	5	404798	5	NULL	NULL	0	NULL	forearm keratin components	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Palmar and plantar keratin contained additional polypeptide chains and had a different size distribution compared with forearm and scalp keratin components .
	manualset3
119545	6	404798	5	NULL	NULL	0	NULL	scalp keratin components	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Palmar and plantar keratin contained additional polypeptide chains and had a different size distribution compared with forearm and scalp keratin components .
	manualset3
119546	1	404799	5	NULL	NULL	0	NULL	Palmitate treatment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Palmitate treatment caused less accumulation of triacylglycerol than did oleate but also induced significant accumulation of both diacylglycerol and ceramide .
	manualset3
119547	2	404799	5	NULL	NULL	0	NULL	accumulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Palmitate treatment caused less accumulation of triacylglycerol than did oleate but also induced significant accumulation of both diacylglycerol and ceramide .
	manualset3
119548	3	404799	5	NULL	NULL	0	NULL	triacylglycerol 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Palmitate treatment caused less accumulation of triacylglycerol than did oleate but also induced significant accumulation of both diacylglycerol and ceramide .
	manualset3
119549	4	404799	5	NULL	NULL	0	NULL	oleate 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Palmitate treatment caused less accumulation of triacylglycerol than did oleate but also induced significant accumulation of both diacylglycerol and ceramide .
	manualset3
119550	5	404799	5	NULL	NULL	0	NULL	accumulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Palmitate treatment caused less accumulation of triacylglycerol than did oleate but also induced significant accumulation of both diacylglycerol and ceramide .
	manualset3
119551	6	404799	5	NULL	NULL	0	NULL	diacylglycerol 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Palmitate treatment caused less accumulation of triacylglycerol than did oleate but also induced significant accumulation of both diacylglycerol and ceramide .
	manualset3
119552	7	404799	5	NULL	NULL	0	NULL	ceramide 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Palmitate treatment caused less accumulation of triacylglycerol than did oleate but also induced significant accumulation of both diacylglycerol and ceramide .
	manualset3
119553	1	404800	5	NULL	NULL	0	NULL	Paludification 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Paludification alters bryophyte abundance and succession , increases soil moisture , reduces soil temperature and nutrient availability , and alters the vertical distribution of roots .
	manualset3
119554	2	404800	5	NULL	NULL	0	NULL	bryophyte abundance 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Paludification alters bryophyte abundance and succession , increases soil moisture , reduces soil temperature and nutrient availability , and alters the vertical distribution of roots .
	manualset3
119555	3	404800	5	NULL	NULL	0	NULL	succession 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Paludification alters bryophyte abundance and succession , increases soil moisture , reduces soil temperature and nutrient availability , and alters the vertical distribution of roots .
	manualset3
119556	4	404800	5	NULL	NULL	0	NULL	soil moisture	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Paludification alters bryophyte abundance and succession , increases soil moisture , reduces soil temperature and nutrient availability , and alters the vertical distribution of roots .
	manualset3
119557	5	404800	5	NULL	NULL	0	NULL	soil temperature	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Paludification alters bryophyte abundance and succession , increases soil moisture , reduces soil temperature and nutrient availability , and alters the vertical distribution of roots .
	manualset3
119558	6	404800	5	NULL	NULL	0	NULL	nutrient availability	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Paludification alters bryophyte abundance and succession , increases soil moisture , reduces soil temperature and nutrient availability , and alters the vertical distribution of roots .
	manualset3
119559	7	404800	5	NULL	NULL	0	NULL	vertical distribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Paludification alters bryophyte abundance and succession , increases soil moisture , reduces soil temperature and nutrient availability , and alters the vertical distribution of roots .
	manualset3
119560	8	404800	5	NULL	NULL	0	NULL	roots 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Paludification alters bryophyte abundance and succession , increases soil moisture , reduces soil temperature and nutrient availability , and alters the vertical distribution of roots .
	manualset3
119561	1	404801	5	NULL	NULL	0	NULL	Pancreatic head carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pancreatic head carcinoma : is pancreatic resection indicated for patients with stage III pancreatic duct cancer ? .
	manualset3
119562	2	404801	5	NULL	NULL	0	NULL	pancreatic resection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pancreatic head carcinoma : is pancreatic resection indicated for patients with stage III pancreatic duct cancer ? .
	manualset3
119563	3	404801	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Pancreatic head carcinoma : is pancreatic resection indicated for patients with stage III pancreatic duct cancer ? .
	manualset3
119564	4	404801	5	NULL	NULL	0	NULL	stage III pancreatic duct cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pancreatic head carcinoma : is pancreatic resection indicated for patients with stage III pancreatic duct cancer ? .
	manualset3
119565	1	404802	5	NULL	NULL	0	NULL	Pancreatic metastasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pancreatic metastasis : sonographic findings .
	manualset3
119566	2	404802	5	NULL	NULL	0	NULL	sonographic findings 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pancreatic metastasis : sonographic findings .
	manualset3
119567	1	404803	5	NULL	NULL	0	NULL	Pancreatic nodules 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Pancreatic nodules were produced in rats by either feeding raw soya flour alone or by injection of azaserine plus raw soya flour feeding .
	manualset3
119568	2	404803	5	NULL	NULL	0	NULL	rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pancreatic nodules were produced in rats by either feeding raw soya flour alone or by injection of azaserine plus raw soya flour feeding .
	manualset3
119569	3	404803	5	NULL	NULL	0	NULL	raw soya flour	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Pancreatic nodules were produced in rats by either feeding raw soya flour alone or by injection of azaserine plus raw soya flour feeding .
	manualset3
119570	4	404803	5	NULL	NULL	0	NULL	azaserine 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Pancreatic nodules were produced in rats by either feeding raw soya flour alone or by injection of azaserine plus raw soya flour feeding .
	manualset3
119571	5	404803	5	NULL	NULL	0	NULL	raw soya flour	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Pancreatic nodules were produced in rats by either feeding raw soya flour alone or by injection of azaserine plus raw soya flour feeding .
	manualset3
119572	1	404804	5	NULL	NULL	0	NULL	Pancreatic pleuropericardial effusions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pancreatic pleuropericardial effusions presenting as tumor of the lung .
	manualset3
119573	2	404804	5	NULL	NULL	0	NULL	tumor 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pancreatic pleuropericardial effusions presenting as tumor of the lung .
	manualset3
119574	3	404804	5	NULL	NULL	0	NULL	lung 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Pancreatic pleuropericardial effusions presenting as tumor of the lung .
	manualset3
119575	1	404805	5	NULL	NULL	0	NULL	Pannexin1 ( Panx1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Pannexin1 ( Panx1 ) , a protein related to the gap junction proteins of invertebrates , forms nonjunctional channels that open upon depolarization and in response to mechanical stretch and purinergic receptor stimulation .
	manualset3
119576	2	404805	5	NULL	NULL	0	NULL	protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Pannexin1 ( Panx1 ) , a protein related to the gap junction proteins of invertebrates , forms nonjunctional channels that open upon depolarization and in response to mechanical stretch and purinergic receptor stimulation .
	manualset3
119577	3	404805	5	NULL	NULL	0	NULL	gap junction proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Pannexin1 ( Panx1 ) , a protein related to the gap junction proteins of invertebrates , forms nonjunctional channels that open upon depolarization and in response to mechanical stretch and purinergic receptor stimulation .
	manualset3
119578	4	404805	5	NULL	NULL	0	NULL	invertebrates 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pannexin1 ( Panx1 ) , a protein related to the gap junction proteins of invertebrates , forms nonjunctional channels that open upon depolarization and in response to mechanical stretch and purinergic receptor stimulation .
	manualset3
119579	5	404805	5	NULL	NULL	0	NULL	nonjunctional channels	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Pannexin1 ( Panx1 ) , a protein related to the gap junction proteins of invertebrates , forms nonjunctional channels that open upon depolarization and in response to mechanical stretch and purinergic receptor stimulation .
	manualset3
119580	6	404805	5	NULL	NULL	0	NULL	depolarization 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pannexin1 ( Panx1 ) , a protein related to the gap junction proteins of invertebrates , forms nonjunctional channels that open upon depolarization and in response to mechanical stretch and purinergic receptor stimulation .
	manualset3
119581	7	404805	5	NULL	NULL	0	NULL	response 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pannexin1 ( Panx1 ) , a protein related to the gap junction proteins of invertebrates , forms nonjunctional channels that open upon depolarization and in response to mechanical stretch and purinergic receptor stimulation .
	manualset3
119582	8	404805	5	NULL	NULL	0	NULL	mechanical stretch	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pannexin1 ( Panx1 ) , a protein related to the gap junction proteins of invertebrates , forms nonjunctional channels that open upon depolarization and in response to mechanical stretch and purinergic receptor stimulation .
	manualset3
119583	9	404805	5	NULL	NULL	0	NULL	purinergic receptor stimulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pannexin1 ( Panx1 ) , a protein related to the gap junction proteins of invertebrates , forms nonjunctional channels that open upon depolarization and in response to mechanical stretch and purinergic receptor stimulation .
	manualset3
119584	1	404806	5	NULL	NULL	0	NULL	Papain-induced symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Papain-induced symptoms included palatal itching , watering itchy eyes , sneezing , rhinorrhea , abdominal cramps , diarrhea , and diaphoresis .
	manualset3
119585	2	404806	5	NULL	NULL	0	NULL	palatal itching	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Papain-induced symptoms included palatal itching , watering itchy eyes , sneezing , rhinorrhea , abdominal cramps , diarrhea , and diaphoresis .
	manualset3
119586	3	404806	5	NULL	NULL	0	NULL	watering itchy eyes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Papain-induced symptoms included palatal itching , watering itchy eyes , sneezing , rhinorrhea , abdominal cramps , diarrhea , and diaphoresis .
	manualset3
119587	4	404806	5	NULL	NULL	0	NULL	sneezing 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Papain-induced symptoms included palatal itching , watering itchy eyes , sneezing , rhinorrhea , abdominal cramps , diarrhea , and diaphoresis .
	manualset3
119588	5	404806	5	NULL	NULL	0	NULL	rhinorrhea 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Papain-induced symptoms included palatal itching , watering itchy eyes , sneezing , rhinorrhea , abdominal cramps , diarrhea , and diaphoresis .
	manualset3
119589	6	404806	5	NULL	NULL	0	NULL	abdominal cramps	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Papain-induced symptoms included palatal itching , watering itchy eyes , sneezing , rhinorrhea , abdominal cramps , diarrhea , and diaphoresis .
	manualset3
119590	7	404806	5	NULL	NULL	0	NULL	diarrhea 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Papain-induced symptoms included palatal itching , watering itchy eyes , sneezing , rhinorrhea , abdominal cramps , diarrhea , and diaphoresis .
	manualset3
119591	8	404806	5	NULL	NULL	0	NULL	diaphoresis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Papain-induced symptoms included palatal itching , watering itchy eyes , sneezing , rhinorrhea , abdominal cramps , diarrhea , and diaphoresis .
	manualset3
119592	1	404807	5	NULL	NULL	0	NULL	Papain ( EC 3.4.22.2 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Papain ( EC 3.4.22.2 ) was photooxidized using methylene blue as a sensitizer .
	manualset3
119593	2	404807	5	NULL	NULL	0	NULL	methylene blue	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Papain ( EC 3.4.22.2 ) was photooxidized using methylene blue as a sensitizer .
	manualset3
119594	3	404807	5	NULL	NULL	0	NULL	sensitizer 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Papain ( EC 3.4.22.2 ) was photooxidized using methylene blue as a sensitizer .
	manualset3
119595	1	404808	5	NULL	NULL	0	NULL	Paper chromatography 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Paper chromatography of oxyacanthine and repandine .
	manualset3
119596	2	404808	5	NULL	NULL	0	NULL	oxyacanthine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Paper chromatography of oxyacanthine and repandine .
	manualset3
119597	3	404808	5	NULL	NULL	0	NULL	repandine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Paper chromatography of oxyacanthine and repandine .
	manualset3
119598	1	404809	5	NULL	NULL	0	NULL	nine-degree-of-freedom ( 9DOF )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A full dimensional , nine-degree-of-freedom ( 9DOF ) , time-dependent quantum dynamics wave packet approach is presented for the study of the H2 + C2H -- ) H+C 2H2 reaction system .
	manualset3
119599	2	404809	5	NULL	NULL	NULL	NULL	time-dependent quantum dynamics wave packet approach	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A full dimensional , nine-degree-of-freedom ( 9DOF ) , time-dependent quantum dynamics wave packet approach is presented for the study of the H2 + C2H -- ) H+C 2H2 reaction system .
	manualset3
119600	3	404809	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A full dimensional , nine-degree-of-freedom ( 9DOF ) , time-dependent quantum dynamics wave packet approach is presented for the study of the H2 + C2H -- ) H+C 2H2 reaction system .
	manualset3
119601	4	404809	5	NULL	NULL	0	NULL	H2 + C2H -- ) H+C 2H2 reaction system	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A full dimensional , nine-degree-of-freedom ( 9DOF ) , time-dependent quantum dynamics wave packet approach is presented for the study of the H2 + C2H -- ) H+C 2H2 reaction system .
	manualset3
119602	1	404810	5	NULL	NULL	0	NULL	Papillomas 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Papillomas frequently recur following surgical resection , however , often necessitating repeated ablative efforts to maintain a patent airway .
	manualset3
119603	2	404810	5	NULL	NULL	0	NULL	surgical resection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Papillomas frequently recur following surgical resection , however , often necessitating repeated ablative efforts to maintain a patent airway .
	manualset3
119604	3	404810	5	NULL	NULL	0	NULL	repeated ablative efforts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Papillomas frequently recur following surgical resection , however , often necessitating repeated ablative efforts to maintain a patent airway .
	manualset3
119605	4	404810	5	NULL	NULL	0	NULL	patent airway	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Papillomas frequently recur following surgical resection , however , often necessitating repeated ablative efforts to maintain a patent airway .
	manualset3
119606	1	404811	5	NULL	NULL	0	NULL	Para-arytenoid cartilage pseudodiverticulum formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Para-arytenoid cartilage pseudodiverticulum formation as a sequela of endotracheal intubation .
	manualset3
119607	2	404811	5	NULL	NULL	0	NULL	sequela 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Para-arytenoid cartilage pseudodiverticulum formation as a sequela of endotracheal intubation .
	manualset3
119608	3	404811	5	NULL	NULL	0	NULL	endotracheal intubation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Para-arytenoid cartilage pseudodiverticulum formation as a sequela of endotracheal intubation .
	manualset3
119609	1	404812	5	NULL	NULL	0	NULL	Paracentesis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Paracentesis results were compared with the results of other tests and surgery in diagnosing hemoperitoneum .
	manualset3
119610	2	404812	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Paracentesis results were compared with the results of other tests and surgery in diagnosing hemoperitoneum .
	manualset3
119611	3	404812	5	NULL	NULL	0	NULL	tests 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Paracentesis results were compared with the results of other tests and surgery in diagnosing hemoperitoneum .
	manualset3
119612	4	404812	5	NULL	NULL	0	NULL	surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Paracentesis results were compared with the results of other tests and surgery in diagnosing hemoperitoneum .
	manualset3
119613	5	404812	5	NULL	NULL	0	NULL	hemoperitoneum 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Paracentesis results were compared with the results of other tests and surgery in diagnosing hemoperitoneum .
	manualset3
119614	1	404813	5	NULL	NULL	0	NULL	Paracoccidioides brasiliensis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Paracoccidioides brasiliensis causes paracoccidioidomycosis ( PCM ) , a systemic mycosis presenting clinical manifestations ranging from mild to severe forms .
	manualset3
119615	2	404813	5	NULL	NULL	0	NULL	paracoccidioidomycosis ( PCM )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Paracoccidioides brasiliensis causes paracoccidioidomycosis ( PCM ) , a systemic mycosis presenting clinical manifestations ranging from mild to severe forms .
	manualset3
119616	3	404813	5	NULL	NULL	0	NULL	systemic mycosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Paracoccidioides brasiliensis causes paracoccidioidomycosis ( PCM ) , a systemic mycosis presenting clinical manifestations ranging from mild to severe forms .
	manualset3
119617	4	404813	5	NULL	NULL	0	NULL	clinical manifestations 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Paracoccidioides brasiliensis causes paracoccidioidomycosis ( PCM ) , a systemic mycosis presenting clinical manifestations ranging from mild to severe forms .
	manualset3
119618	5	404813	5	NULL	NULL	0	NULL	mild to severe forms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Paracoccidioides brasiliensis causes paracoccidioidomycosis ( PCM ) , a systemic mycosis presenting clinical manifestations ranging from mild to severe forms .
	manualset3
119619	1	404814	5	NULL	NULL	0	NULL	Paradontitis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Paradontitis is one of more risk factors of cardiovascular diseases ) .
	manualset3
119620	2	404814	5	NULL	NULL	0	NULL	risk factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Paradontitis is one of more risk factors of cardiovascular diseases ) .
	manualset3
119621	3	404814	5	NULL	NULL	0	NULL	cardiovascular diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Paradontitis is one of more risk factors of cardiovascular diseases ) .
	manualset3
119622	1	404815	5	NULL	NULL	0	NULL	Paradoxical conditioning	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Paradoxical conditioning of the plasma copper and corticosterone responses to bacterial endotoxin .
	manualset3
119623	2	404815	5	NULL	NULL	0	NULL	plasma copper	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Paradoxical conditioning of the plasma copper and corticosterone responses to bacterial endotoxin .
	manualset3
119624	3	404815	5	NULL	NULL	0	NULL	corticosterone responses	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Paradoxical conditioning of the plasma copper and corticosterone responses to bacterial endotoxin .
	manualset3
119625	4	404815	5	NULL	NULL	0	NULL	bacterial endotoxin 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Paradoxical conditioning of the plasma copper and corticosterone responses to bacterial endotoxin .
	manualset3
119626	1	404816	5	NULL	NULL	0	NULL	immunoprecipitated CFTR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Paradoxically , immunoprecipitated CFTR or CF-2 , a cloned R domain fragment of CFTR ( amino acids 645-835 ) could be phosphorylated to a similar extent with only minor kinetic differences by both isotypes of cGK .
	manualset3
119627	2	404816	5	NULL	NULL	0	NULL	CF-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Paradoxically , immunoprecipitated CFTR or CF-2 , a cloned R domain fragment of CFTR ( amino acids 645-835 ) could be phosphorylated to a similar extent with only minor kinetic differences by both isotypes of cGK .
	manualset3
119628	3	404816	5	NULL	NULL	0	NULL	R domain fragment of CFTR ( amino acids 645-835 )	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Paradoxically , immunoprecipitated CFTR or CF-2 , a cloned R domain fragment of CFTR ( amino acids 645-835 ) could be phosphorylated to a similar extent with only minor kinetic differences by both isotypes of cGK .
	manualset3
119629	4	404816	5	NULL	NULL	0	NULL	kinetic differences	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Paradoxically , immunoprecipitated CFTR or CF-2 , a cloned R domain fragment of CFTR ( amino acids 645-835 ) could be phosphorylated to a similar extent with only minor kinetic differences by both isotypes of cGK .
	manualset3
119630	5	404816	5	NULL	NULL	0	NULL	isotypes of cGK 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Paradoxically , immunoprecipitated CFTR or CF-2 , a cloned R domain fragment of CFTR ( amino acids 645-835 ) could be phosphorylated to a similar extent with only minor kinetic differences by both isotypes of cGK .
	manualset3
119631	1	404817	5	NULL	NULL	0	NULL	Parallel detection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel detection of transduced T lymphocytes after immunogene therapy of renal cell cancer by flow cytometry and real-time polymerase chain reaction : implications for loss of transgene expression .
	manualset3
119632	2	404817	5	NULL	NULL	0	NULL	transduced T lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel detection of transduced T lymphocytes after immunogene therapy of renal cell cancer by flow cytometry and real-time polymerase chain reaction : implications for loss of transgene expression .
	manualset3
119633	3	404817	5	NULL	NULL	0	NULL	immunogene therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel detection of transduced T lymphocytes after immunogene therapy of renal cell cancer by flow cytometry and real-time polymerase chain reaction : implications for loss of transgene expression .
	manualset3
119634	4	404817	5	NULL	NULL	0	NULL	renal cell cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel detection of transduced T lymphocytes after immunogene therapy of renal cell cancer by flow cytometry and real-time polymerase chain reaction : implications for loss of transgene expression .
	manualset3
119635	5	404817	5	NULL	NULL	0	NULL	flow cytometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel detection of transduced T lymphocytes after immunogene therapy of renal cell cancer by flow cytometry and real-time polymerase chain reaction : implications for loss of transgene expression .
	manualset3
119636	6	404817	5	NULL	NULL	0	NULL	real-time polymerase chain reaction 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel detection of transduced T lymphocytes after immunogene therapy of renal cell cancer by flow cytometry and real-time polymerase chain reaction : implications for loss of transgene expression .
	manualset3
119637	7	404817	5	NULL	NULL	0	NULL	implications 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel detection of transduced T lymphocytes after immunogene therapy of renal cell cancer by flow cytometry and real-time polymerase chain reaction : implications for loss of transgene expression .
	manualset3
119638	8	404817	5	NULL	NULL	0	NULL	loss 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel detection of transduced T lymphocytes after immunogene therapy of renal cell cancer by flow cytometry and real-time polymerase chain reaction : implications for loss of transgene expression .
	manualset3
119639	9	404817	5	NULL	NULL	0	NULL	transgene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel detection of transduced T lymphocytes after immunogene therapy of renal cell cancer by flow cytometry and real-time polymerase chain reaction : implications for loss of transgene expression .
	manualset3
119640	1	404818	5	NULL	NULL	0	NULL	Parallel studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel studies of lipid bilayer vesicles using a dye binding assay to detect fibril formation and electron microscopy to examine morphology demonstrated that Abeta42 pretreatment of oxidatively damaged membranes promoted the formation of mature Abeta40 amyloid fibrils .
	manualset3
119641	2	404818	5	NULL	NULL	0	NULL	lipid bilayer vesicles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel studies of lipid bilayer vesicles using a dye binding assay to detect fibril formation and electron microscopy to examine morphology demonstrated that Abeta42 pretreatment of oxidatively damaged membranes promoted the formation of mature Abeta40 amyloid fibrils .
	manualset3
119642	3	404818	5	NULL	NULL	0	NULL	dye binding assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel studies of lipid bilayer vesicles using a dye binding assay to detect fibril formation and electron microscopy to examine morphology demonstrated that Abeta42 pretreatment of oxidatively damaged membranes promoted the formation of mature Abeta40 amyloid fibrils .
	manualset3
119643	4	404818	5	NULL	NULL	0	NULL	fibril formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel studies of lipid bilayer vesicles using a dye binding assay to detect fibril formation and electron microscopy to examine morphology demonstrated that Abeta42 pretreatment of oxidatively damaged membranes promoted the formation of mature Abeta40 amyloid fibrils .
	manualset3
119644	5	404818	5	NULL	NULL	0	NULL	electron microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel studies of lipid bilayer vesicles using a dye binding assay to detect fibril formation and electron microscopy to examine morphology demonstrated that Abeta42 pretreatment of oxidatively damaged membranes promoted the formation of mature Abeta40 amyloid fibrils .
	manualset3
119645	6	404818	5	NULL	NULL	0	NULL	morphology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel studies of lipid bilayer vesicles using a dye binding assay to detect fibril formation and electron microscopy to examine morphology demonstrated that Abeta42 pretreatment of oxidatively damaged membranes promoted the formation of mature Abeta40 amyloid fibrils .
	manualset3
119646	7	404818	5	NULL	NULL	0	NULL	Abeta42 pretreatment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel studies of lipid bilayer vesicles using a dye binding assay to detect fibril formation and electron microscopy to examine morphology demonstrated that Abeta42 pretreatment of oxidatively damaged membranes promoted the formation of mature Abeta40 amyloid fibrils .
	manualset3
119647	8	404818	5	NULL	NULL	0	NULL	oxidatively damaged membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel studies of lipid bilayer vesicles using a dye binding assay to detect fibril formation and electron microscopy to examine morphology demonstrated that Abeta42 pretreatment of oxidatively damaged membranes promoted the formation of mature Abeta40 amyloid fibrils .
	manualset3
119648	9	404818	5	NULL	NULL	0	NULL	formation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel studies of lipid bilayer vesicles using a dye binding assay to detect fibril formation and electron microscopy to examine morphology demonstrated that Abeta42 pretreatment of oxidatively damaged membranes promoted the formation of mature Abeta40 amyloid fibrils .
	manualset3
119649	10	404818	5	NULL	NULL	0	NULL	mature Abeta40 amyloid fibrils	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel studies of lipid bilayer vesicles using a dye binding assay to detect fibril formation and electron microscopy to examine morphology demonstrated that Abeta42 pretreatment of oxidatively damaged membranes promoted the formation of mature Abeta40 amyloid fibrils .
	manualset3
119650	1	404819	5	NULL	NULL	0	NULL	Parallel traveling-wave MRI	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel traveling-wave MRI : A feasibility study .
	manualset3
119651	2	404819	5	NULL	NULL	0	NULL	feasibility study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel traveling-wave MRI : A feasibility study .
	manualset3
119652	1	404820	5	NULL	NULL	0	NULL	function 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A function of the apex as a sink for cytokinins may also be involved in the control mechanism .
	manualset3
119653	2	404820	5	NULL	NULL	0	NULL	apex 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A function of the apex as a sink for cytokinins may also be involved in the control mechanism .
	manualset3
119654	3	404820	5	NULL	NULL	0	NULL	sink 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A function of the apex as a sink for cytokinins may also be involved in the control mechanism .
	manualset3
119655	4	404820	5	NULL	NULL	0	NULL	cytokinins 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A function of the apex as a sink for cytokinins may also be involved in the control mechanism .
	manualset3
119656	5	404820	5	NULL	NULL	0	NULL	control mechanism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A function of the apex as a sink for cytokinins may also be involved in the control mechanism .
	manualset3
119657	1	404821	5	NULL	NULL	0	NULL	Parallel upstream/downstream patterns	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel upstream/downstream patterns of morphological adaptation in response to selection pressures reported in P. reticulata within Trinidad rivers appears to persist across the natural range .
	manualset3
119658	2	404821	5	NULL	NULL	0	NULL	morphological adaptation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel upstream/downstream patterns of morphological adaptation in response to selection pressures reported in P. reticulata within Trinidad rivers appears to persist across the natural range .
	manualset3
119659	3	404821	5	NULL	NULL	0	NULL	response 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel upstream/downstream patterns of morphological adaptation in response to selection pressures reported in P. reticulata within Trinidad rivers appears to persist across the natural range .
	manualset3
119660	4	404821	5	NULL	NULL	NULL	NULL	selection pressures	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Parallel upstream/downstream patterns of morphological adaptation in response to selection pressures reported in P. reticulata within Trinidad rivers appears to persist across the natural range .
	manualset3
119661	5	404821	5	NULL	NULL	0	NULL	P. reticulata 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel upstream/downstream patterns of morphological adaptation in response to selection pressures reported in P. reticulata within Trinidad rivers appears to persist across the natural range .
	manualset3
119662	6	404821	5	NULL	NULL	0	NULL	Trinidad rivers 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel upstream/downstream patterns of morphological adaptation in response to selection pressures reported in P. reticulata within Trinidad rivers appears to persist across the natural range .
	manualset3
119663	7	404821	5	NULL	NULL	0	NULL	natural range	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel upstream/downstream patterns of morphological adaptation in response to selection pressures reported in P. reticulata within Trinidad rivers appears to persist across the natural range .
	manualset3
119664	1	404822	5	NULL	NULL	0	NULL	Parallel experiments 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel experiments revealed that when the trk receptors were inhibited by K252a or the action of BDNF was inhibited by a neutralizing anti-BDNF antibody , the effects of SMI on the A ( 25-35 ) - induced neurodegeneration in rat cortical neurons were almost completely abolished .
	manualset3
119665	2	404822	5	NULL	NULL	0	NULL	trk receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel experiments revealed that when the trk receptors were inhibited by K252a or the action of BDNF was inhibited by a neutralizing anti-BDNF antibody , the effects of SMI on the A ( 25-35 ) - induced neurodegeneration in rat cortical neurons were almost completely abolished .
	manualset3
119666	3	404822	5	NULL	NULL	0	NULL	K252a 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel experiments revealed that when the trk receptors were inhibited by K252a or the action of BDNF was inhibited by a neutralizing anti-BDNF antibody , the effects of SMI on the A ( 25-35 ) - induced neurodegeneration in rat cortical neurons were almost completely abolished .
	manualset3
119667	4	404822	5	NULL	NULL	0	NULL	action 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel experiments revealed that when the trk receptors were inhibited by K252a or the action of BDNF was inhibited by a neutralizing anti-BDNF antibody , the effects of SMI on the A ( 25-35 ) - induced neurodegeneration in rat cortical neurons were almost completely abolished .
	manualset3
119668	5	404822	5	NULL	NULL	0	NULL	BDNF 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel experiments revealed that when the trk receptors were inhibited by K252a or the action of BDNF was inhibited by a neutralizing anti-BDNF antibody , the effects of SMI on the A ( 25-35 ) - induced neurodegeneration in rat cortical neurons were almost completely abolished .
	manualset3
119669	6	404822	5	NULL	NULL	0	NULL	anti-BDNF antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel experiments revealed that when the trk receptors were inhibited by K252a or the action of BDNF was inhibited by a neutralizing anti-BDNF antibody , the effects of SMI on the A ( 25-35 ) - induced neurodegeneration in rat cortical neurons were almost completely abolished .
	manualset3
119670	7	404822	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel experiments revealed that when the trk receptors were inhibited by K252a or the action of BDNF was inhibited by a neutralizing anti-BDNF antibody , the effects of SMI on the A ( 25-35 ) - induced neurodegeneration in rat cortical neurons were almost completely abolished .
	manualset3
119671	8	404822	5	NULL	NULL	0	NULL	SMI 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel experiments revealed that when the trk receptors were inhibited by K252a or the action of BDNF was inhibited by a neutralizing anti-BDNF antibody , the effects of SMI on the A ( 25-35 ) - induced neurodegeneration in rat cortical neurons were almost completely abolished .
	manualset3
119672	9	404822	5	NULL	NULL	0	NULL	A ( 25-35 ) - induced neurodegeneration	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel experiments revealed that when the trk receptors were inhibited by K252a or the action of BDNF was inhibited by a neutralizing anti-BDNF antibody , the effects of SMI on the A ( 25-35 ) - induced neurodegeneration in rat cortical neurons were almost completely abolished .
	manualset3
119673	10	404822	5	NULL	NULL	0	NULL	rat cortical neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel experiments revealed that when the trk receptors were inhibited by K252a or the action of BDNF was inhibited by a neutralizing anti-BDNF antibody , the effects of SMI on the A ( 25-35 ) - induced neurodegeneration in rat cortical neurons were almost completely abolished .
	manualset3
119674	1	404823	5	NULL	NULL	0	NULL	Parameter-free theory 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Parameter-free theory shows that the existing experimental techniques permit observation of the driven coupled oscillations of the spin and the cantilever , as well as of the splitting of the mechanical modes of the cantilever caused by spin tunneling .
	manualset3
119675	2	404823	5	NULL	NULL	0	NULL	existing experimental techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parameter-free theory shows that the existing experimental techniques permit observation of the driven coupled oscillations of the spin and the cantilever , as well as of the splitting of the mechanical modes of the cantilever caused by spin tunneling .
	manualset3
119676	3	404823	5	NULL	NULL	0	NULL	observation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Parameter-free theory shows that the existing experimental techniques permit observation of the driven coupled oscillations of the spin and the cantilever , as well as of the splitting of the mechanical modes of the cantilever caused by spin tunneling .
	manualset3
119677	4	404823	5	NULL	NULL	0	NULL	driven coupled oscillations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Parameter-free theory shows that the existing experimental techniques permit observation of the driven coupled oscillations of the spin and the cantilever , as well as of the splitting of the mechanical modes of the cantilever caused by spin tunneling .
	manualset3
119678	5	404823	5	NULL	NULL	0	NULL	spin 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Parameter-free theory shows that the existing experimental techniques permit observation of the driven coupled oscillations of the spin and the cantilever , as well as of the splitting of the mechanical modes of the cantilever caused by spin tunneling .
	manualset3
119679	6	404823	5	NULL	NULL	0	NULL	cantilever 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Parameter-free theory shows that the existing experimental techniques permit observation of the driven coupled oscillations of the spin and the cantilever , as well as of the splitting of the mechanical modes of the cantilever caused by spin tunneling .
	manualset3
119680	7	404823	5	NULL	NULL	NULL	NULL	mechanical modes 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Parameter-free theory shows that the existing experimental techniques permit observation of the driven coupled oscillations of the spin and the cantilever , as well as of the splitting of the mechanical modes of the cantilever caused by spin tunneling .
	manualset3
119681	8	404823	5	NULL	NULL	0	NULL	cantilever 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Parameter-free theory shows that the existing experimental techniques permit observation of the driven coupled oscillations of the spin and the cantilever , as well as of the splitting of the mechanical modes of the cantilever caused by spin tunneling .
	manualset3
122300	9	404823	5	NULL	NULL	0	NULL	spin tunneling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Parameter-free theory shows that the existing experimental techniques permit observation of the driven coupled oscillations of the spin and the cantilever , as well as of the splitting of the mechanical modes of the cantilever caused by spin tunneling .
	manualset3
119682	1	404824	5	NULL	NULL	0	NULL	Parameters 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parameters characterizing EGFR and HER2 interactions were determined using experimental data obtained from mammary epithelial cells constructed to express different levels of HER2 , enabling us to estimate receptor-specific internalization rate constants and dimer uncoupling rate constants .
	manualset3
119683	2	404824	5	NULL	NULL	0	NULL	EGFR and HER2 interactions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Parameters characterizing EGFR and HER2 interactions were determined using experimental data obtained from mammary epithelial cells constructed to express different levels of HER2 , enabling us to estimate receptor-specific internalization rate constants and dimer uncoupling rate constants .
	manualset3
119684	3	404824	5	NULL	NULL	0	NULL	experimental data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Parameters characterizing EGFR and HER2 interactions were determined using experimental data obtained from mammary epithelial cells constructed to express different levels of HER2 , enabling us to estimate receptor-specific internalization rate constants and dimer uncoupling rate constants .
	manualset3
119685	4	404824	5	NULL	NULL	0	NULL	mammary epithelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Parameters characterizing EGFR and HER2 interactions were determined using experimental data obtained from mammary epithelial cells constructed to express different levels of HER2 , enabling us to estimate receptor-specific internalization rate constants and dimer uncoupling rate constants .
	manualset3
119686	5	404824	5	NULL	NULL	0	NULL	different levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parameters characterizing EGFR and HER2 interactions were determined using experimental data obtained from mammary epithelial cells constructed to express different levels of HER2 , enabling us to estimate receptor-specific internalization rate constants and dimer uncoupling rate constants .
	manualset3
119687	6	404824	5	NULL	NULL	0	NULL	HER2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Parameters characterizing EGFR and HER2 interactions were determined using experimental data obtained from mammary epithelial cells constructed to express different levels of HER2 , enabling us to estimate receptor-specific internalization rate constants and dimer uncoupling rate constants .
	manualset3
119688	7	404824	5	NULL	NULL	NULL	NULL	receptor-specific internalization rate constants	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Parameters characterizing EGFR and HER2 interactions were determined using experimental data obtained from mammary epithelial cells constructed to express different levels of HER2 , enabling us to estimate receptor-specific internalization rate constants and dimer uncoupling rate constants .
	manualset3
119689	8	404824	5	NULL	NULL	0	NULL	dimer uncoupling rate constants	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parameters characterizing EGFR and HER2 interactions were determined using experimental data obtained from mammary epithelial cells constructed to express different levels of HER2 , enabling us to estimate receptor-specific internalization rate constants and dimer uncoupling rate constants .
	manualset3
119690	1	404825	5	NULL	NULL	0	NULL	Parameters 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parameters measured included performance , organ weights , and plasma chemistry .
	manualset3
119691	2	404825	5	NULL	NULL	0	NULL	performance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Parameters measured included performance , organ weights , and plasma chemistry .
	manualset3
119692	3	404825	5	NULL	NULL	0	NULL	organ weights	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parameters measured included performance , organ weights , and plasma chemistry .
	manualset3
119693	4	404825	5	NULL	NULL	0	NULL	plasma chemistry 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parameters measured included performance , organ weights , and plasma chemistry .
	manualset3
119694	1	404826	5	NULL	NULL	0	NULL	functional FXR binding site	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A functional FXR binding site was identified in the Abcg5 gene promoter .
	manualset3
119695	2	404826	5	NULL	NULL	0	NULL	Abcg5 gene promoter 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A functional FXR binding site was identified in the Abcg5 gene promoter .
	manualset3
119696	1	404827	5	NULL	NULL	0	NULL	Parameters 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parameters of the orientation/positioning of the tibial component : Varus/valgus , posterior tibial slope and rotation were measured with both modalities .
	manualset3
119697	2	404827	5	NULL	NULL	0	NULL	orientation/positioning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Parameters of the orientation/positioning of the tibial component : Varus/valgus , posterior tibial slope and rotation were measured with both modalities .
	manualset3
119698	3	404827	5	NULL	NULL	0	NULL	tibial component	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Parameters of the orientation/positioning of the tibial component : Varus/valgus , posterior tibial slope and rotation were measured with both modalities .
	manualset3
119699	4	404827	5	NULL	NULL	0	NULL	Varus/valgus	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parameters of the orientation/positioning of the tibial component : Varus/valgus , posterior tibial slope and rotation were measured with both modalities .
	manualset3
119700	5	404827	5	NULL	NULL	0	NULL	posterior tibial slope	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parameters of the orientation/positioning of the tibial component : Varus/valgus , posterior tibial slope and rotation were measured with both modalities .
	manualset3
119701	6	404827	5	NULL	NULL	0	NULL	rotation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Parameters of the orientation/positioning of the tibial component : Varus/valgus , posterior tibial slope and rotation were measured with both modalities .
	manualset3
119702	7	404827	5	NULL	NULL	0	NULL	modalities 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parameters of the orientation/positioning of the tibial component : Varus/valgus , posterior tibial slope and rotation were measured with both modalities .
	manualset3
119703	1	404828	5	NULL	NULL	0	NULL	Parasite lactate dehydrogenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Parasite lactate dehydrogenase exhibits high catalytic efficiency in the reduction of pyruvate , kcat/Km = 9.0 x 10 ( 8 ) min ( -1 ) M ( -1 ) .
	manualset3
119704	2	404828	5	NULL	NULL	0	NULL	high catalytic efficiency	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Parasite lactate dehydrogenase exhibits high catalytic efficiency in the reduction of pyruvate , kcat/Km = 9.0 x 10 ( 8 ) min ( -1 ) M ( -1 ) .
	manualset3
119705	3	404828	5	NULL	NULL	0	NULL	reduction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Parasite lactate dehydrogenase exhibits high catalytic efficiency in the reduction of pyruvate , kcat/Km = 9.0 x 10 ( 8 ) min ( -1 ) M ( -1 ) .
	manualset3
119706	4	404828	5	NULL	NULL	0	NULL	pyruvate 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Parasite lactate dehydrogenase exhibits high catalytic efficiency in the reduction of pyruvate , kcat/Km = 9.0 x 10 ( 8 ) min ( -1 ) M ( -1 ) .
	manualset3
119707	5	404828	5	NULL	NULL	0	NULL	 kcat/Km = 9.0 x 10 ( 8 ) min ( -1 ) M ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Parasite lactate dehydrogenase exhibits high catalytic efficiency in the reduction of pyruvate , kcat/Km = 9.0 x 10 ( 8 ) min ( -1 ) M ( -1 ) .
	manualset3
119708	1	404829	5	NULL	NULL	0	NULL	Parathyroid hormone-related peptide ( PTHrP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Parathyroid hormone-related peptide ( PTHrP ) is expressed throughout the cardiovascular system including coronary endothelial cells .
	manualset3
119709	2	404829	5	NULL	NULL	0	NULL	cardiovascular system	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Parathyroid hormone-related peptide ( PTHrP ) is expressed throughout the cardiovascular system including coronary endothelial cells .
	manualset3
119710	3	404829	5	NULL	NULL	0	NULL	coronary endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Parathyroid hormone-related peptide ( PTHrP ) is expressed throughout the cardiovascular system including coronary endothelial cells .
	manualset3
119711	1	404830	5	NULL	NULL	0	NULL	Parenchymal changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Parenchymal changes related to plasma protein extravasation in experimental seizures .
	manualset3
119712	2	404830	5	NULL	NULL	0	NULL	plasma protein extravasation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Parenchymal changes related to plasma protein extravasation in experimental seizures .
	manualset3
119713	3	404830	5	NULL	NULL	0	NULL	experimental seizures	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parenchymal changes related to plasma protein extravasation in experimental seizures .
	manualset3
119714	1	404831	5	NULL	NULL	0	NULL	Parent-adolescent communication	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Parent-adolescent communication about sexual intercourse : an analysis of maternal reluctance to communicate .
	manualset3
119715	2	404831	5	NULL	NULL	0	NULL	sexual intercourse	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Parent-adolescent communication about sexual intercourse : an analysis of maternal reluctance to communicate .
	manualset3
119716	3	404831	5	NULL	NULL	0	NULL	analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parent-adolescent communication about sexual intercourse : an analysis of maternal reluctance to communicate .
	manualset3
119717	4	404831	5	NULL	NULL	0	NULL	maternal reluctance	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Parent-adolescent communication about sexual intercourse : an analysis of maternal reluctance to communicate .
	manualset3
119750	1	404832	5	NULL	NULL	0	NULL	Parentages	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Parentages of the study population were efficiently discriminated by genotyping 17 microsatellite loci .
	manualset3
119751	2	404832	5	NULL	NULL	0	NULL	study population	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Parentages of the study population were efficiently discriminated by genotyping 17 microsatellite loci .
	manualset3
119752	3	404832	5	NULL	NULL	0	NULL	genotyping	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parentages of the study population were efficiently discriminated by genotyping 17 microsatellite loci .
	manualset3
119753	4	404832	5	NULL	NULL	0	NULL	17 microsatellite loci	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Parentages of the study population were efficiently discriminated by genotyping 17 microsatellite loci .
	manualset3
119754	1	404833	5	NULL	NULL	0	NULL	Parental attitudes	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Parental attitudes and childhood immunization .
	manualset3
119755	2	404833	5	NULL	NULL	0	NULL	childhood immunization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Parental attitudes and childhood immunization .
	manualset3
119756	1	404834	5	NULL	NULL	0	NULL	Parents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Parents ' heightened response to own infant accords with evolutionary models underscoring the need to direct resources to the survival and well being of one 's own offspring .
	manualset3
119757	2	404834	5	NULL	NULL	0	NULL	heightened response	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Parents ' heightened response to own infant accords with evolutionary models underscoring the need to direct resources to the survival and well being of one 's own offspring .
	manualset3
119758	3	404834	5	NULL	NULL	0	NULL	infant accords	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Parents ' heightened response to own infant accords with evolutionary models underscoring the need to direct resources to the survival and well being of one 's own offspring .
	manualset3
119759	4	404834	5	NULL	NULL	0	NULL	evolutionary models 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Parents ' heightened response to own infant accords with evolutionary models underscoring the need to direct resources to the survival and well being of one 's own offspring .
	manualset3
119760	5	404834	5	NULL	NULL	0	NULL	resources	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parents ' heightened response to own infant accords with evolutionary models underscoring the need to direct resources to the survival and well being of one 's own offspring .
	manualset3
119761	6	404834	5	NULL	NULL	0	NULL	survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Parents ' heightened response to own infant accords with evolutionary models underscoring the need to direct resources to the survival and well being of one 's own offspring .
	manualset3
119762	7	404834	5	NULL	NULL	0	NULL	well being	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Parents ' heightened response to own infant accords with evolutionary models underscoring the need to direct resources to the survival and well being of one 's own offspring .
	manualset3
119763	8	404834	5	NULL	NULL	0	NULL	own offspring	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Parents ' heightened response to own infant accords with evolutionary models underscoring the need to direct resources to the survival and well being of one 's own offspring .
	manualset3
122301	9	404834	5	NULL	NULL	0	NULL	need	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Parents ' heightened response to own infant accords with evolutionary models underscoring the need to direct resources to the survival and well being of one 's own offspring .
	manualset3
119764	1	404835	5	NULL	NULL	0	NULL	Parents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Parents who have a newborn requiring intensive care can have a disruption or delay in this attachment process .
	manualset3
119765	2	404835	5	NULL	NULL	0	NULL	newborn	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Parents who have a newborn requiring intensive care can have a disruption or delay in this attachment process .
	manualset3
119766	3	404835	5	NULL	NULL	0	NULL	intensive care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Parents who have a newborn requiring intensive care can have a disruption or delay in this attachment process .
	manualset3
119767	4	404835	5	NULL	NULL	0	NULL	disruption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Parents who have a newborn requiring intensive care can have a disruption or delay in this attachment process .
	manualset3
119768	5	404835	5	NULL	NULL	0	NULL	delay	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Parents who have a newborn requiring intensive care can have a disruption or delay in this attachment process .
	manualset3
119769	6	404835	5	NULL	NULL	NULL	NULL	attachment process	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Parents who have a newborn requiring intensive care can have a disruption or delay in this attachment process .
	manualset3
119770	1	404836	5	NULL	NULL	0	NULL	Parietal cell structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parietal cell structure during inhibition of acid secretion .
	manualset3
119771	2	404836	5	NULL	NULL	0	NULL	inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Parietal cell structure during inhibition of acid secretion .
	manualset3
119772	3	404836	5	NULL	NULL	0	NULL	acid secretion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Parietal cell structure during inhibition of acid secretion .
	manualset3
119773	1	404837	5	NULL	NULL	0	NULL	Parkinson 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Parkinson 's disease affects several neuronal structures outside the substantia nigra , among which is the enteric nervous system .
	manualset3
119774	2	404837	5	NULL	NULL	0	NULL	neuronal structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parkinson 's disease affects several neuronal structures outside the substantia nigra , among which is the enteric nervous system .
	manualset3
119775	3	404837	5	NULL	NULL	0	NULL	substantia nigra	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Parkinson 's disease affects several neuronal structures outside the substantia nigra , among which is the enteric nervous system .
	manualset3
119776	4	404837	5	NULL	NULL	0	NULL	nervous system	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Parkinson 's disease affects several neuronal structures outside the substantia nigra , among which is the enteric nervous system .
	manualset3
120006	1	404838	5	NULL	NULL	0	NULL	Parous Merino ewes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Parous Merino ewes were maintained outdoors in feedlots during the beginning of the spontaneous breeding season and fed a maintenance ration of wheaten hay .
	manualset3
120007	2	404838	5	NULL	NULL	0	NULL	outdoors 	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Parous Merino ewes were maintained outdoors in feedlots during the beginning of the spontaneous breeding season and fed a maintenance ration of wheaten hay .
	manualset3
120008	3	404838	5	NULL	NULL	0	NULL	feedlots 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Parous Merino ewes were maintained outdoors in feedlots during the beginning of the spontaneous breeding season and fed a maintenance ration of wheaten hay .
	manualset3
120014	4	404838	5	NULL	NULL	0	NULL	beginning 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Parous Merino ewes were maintained outdoors in feedlots during the beginning of the spontaneous breeding season and fed a maintenance ration of wheaten hay .
	manualset3
120015	5	404838	5	NULL	NULL	0	NULL	spontaneous breeding season	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Parous Merino ewes were maintained outdoors in feedlots during the beginning of the spontaneous breeding season and fed a maintenance ration of wheaten hay .
	manualset3
120016	6	404838	5	NULL	NULL	0	NULL	maintenance ration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parous Merino ewes were maintained outdoors in feedlots during the beginning of the spontaneous breeding season and fed a maintenance ration of wheaten hay .
	manualset3
120042	7	404838	5	NULL	NULL	0	NULL	wheaten hay	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Parous Merino ewes were maintained outdoors in feedlots during the beginning of the spontaneous breeding season and fed a maintenance ration of wheaten hay .
	manualset3
120045	1	404839	5	NULL	NULL	0	NULL	functionally graded coating	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A functionally graded coating , consisting of a 6P68 interfacial layer and an H12 surface layer , was developed to provide a coating with high adhesive strength coupled with rapid in vitro bioactivity .
	manualset3
120049	2	404839	5	NULL	NULL	0	NULL	6P68 interfacial layer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A functionally graded coating , consisting of a 6P68 interfacial layer and an H12 surface layer , was developed to provide a coating with high adhesive strength coupled with rapid in vitro bioactivity .
	manualset3
120050	3	404839	5	NULL	NULL	0	NULL	 H12 surface layer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A functionally graded coating , consisting of a 6P68 interfacial layer and an H12 surface layer , was developed to provide a coating with high adhesive strength coupled with rapid in vitro bioactivity .
	manualset3
120051	4	404839	5	NULL	NULL	0	NULL	coating 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A functionally graded coating , consisting of a 6P68 interfacial layer and an H12 surface layer , was developed to provide a coating with high adhesive strength coupled with rapid in vitro bioactivity .
	manualset3
120052	5	404839	5	NULL	NULL	0	NULL	high adhesive strength	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A functionally graded coating , consisting of a 6P68 interfacial layer and an H12 surface layer , was developed to provide a coating with high adhesive strength coupled with rapid in vitro bioactivity .
	manualset3
120053	6	404839	5	NULL	NULL	0	NULL	rapid in vitro bioactivity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A functionally graded coating , consisting of a 6P68 interfacial layer and an H12 surface layer , was developed to provide a coating with high adhesive strength coupled with rapid in vitro bioactivity .
	manualset3
120063	1	404840	5	NULL	NULL	NULL	NULL	Paroxysmal hemicrania	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Paroxysmal hemicrania has been described as an excruciating unilateral pain , which is usually ocular and frontotemporal with short-lasting ( 2-45 min ) , frequent attacks ( usually more than five per day ) ; with marked autonomic features ( rhinorrhoea , nasal congestion , conjunctival injection , lacrimation ) and unilateral to the pain .
	manualset3
120064	2	404840	5	NULL	NULL	0	NULL	excruciating unilateral pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Paroxysmal hemicrania has been described as an excruciating unilateral pain , which is usually ocular and frontotemporal with short-lasting ( 2-45 min ) , frequent attacks ( usually more than five per day ) ; with marked autonomic features ( rhinorrhoea , nasal congestion , conjunctival injection , lacrimation ) and unilateral to the pain .
	manualset3
120067	3	404840	5	NULL	NULL	NULL	NULL	 2-45 min 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Paroxysmal hemicrania has been described as an excruciating unilateral pain , which is usually ocular and frontotemporal with short-lasting ( 2-45 min ) , frequent attacks ( usually more than five per day ) ; with marked autonomic features ( rhinorrhoea , nasal congestion , conjunctival injection , lacrimation ) and unilateral to the pain .
	manualset3
120068	4	404840	5	NULL	NULL	0	NULL	frequent attacks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Paroxysmal hemicrania has been described as an excruciating unilateral pain , which is usually ocular and frontotemporal with short-lasting ( 2-45 min ) , frequent attacks ( usually more than five per day ) ; with marked autonomic features ( rhinorrhoea , nasal congestion , conjunctival injection , lacrimation ) and unilateral to the pain .
	manualset3
120071	5	404840	5	NULL	NULL	0	NULL	five 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Paroxysmal hemicrania has been described as an excruciating unilateral pain , which is usually ocular and frontotemporal with short-lasting ( 2-45 min ) , frequent attacks ( usually more than five per day ) ; with marked autonomic features ( rhinorrhoea , nasal congestion , conjunctival injection , lacrimation ) and unilateral to the pain .
	manualset3
120072	6	404840	5	NULL	NULL	0	NULL	day 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Paroxysmal hemicrania has been described as an excruciating unilateral pain , which is usually ocular and frontotemporal with short-lasting ( 2-45 min ) , frequent attacks ( usually more than five per day ) ; with marked autonomic features ( rhinorrhoea , nasal congestion , conjunctival injection , lacrimation ) and unilateral to the pain .
	manualset3
120074	7	404840	5	NULL	NULL	0	NULL	autonomic features 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Paroxysmal hemicrania has been described as an excruciating unilateral pain , which is usually ocular and frontotemporal with short-lasting ( 2-45 min ) , frequent attacks ( usually more than five per day ) ; with marked autonomic features ( rhinorrhoea , nasal congestion , conjunctival injection , lacrimation ) and unilateral to the pain .
	manualset3
120075	8	404840	5	NULL	NULL	0	NULL	nasal congestion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Paroxysmal hemicrania has been described as an excruciating unilateral pain , which is usually ocular and frontotemporal with short-lasting ( 2-45 min ) , frequent attacks ( usually more than five per day ) ; with marked autonomic features ( rhinorrhoea , nasal congestion , conjunctival injection , lacrimation ) and unilateral to the pain .
	manualset3
120080	9	404840	5	NULL	NULL	0	NULL	conjunctival injection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Paroxysmal hemicrania has been described as an excruciating unilateral pain , which is usually ocular and frontotemporal with short-lasting ( 2-45 min ) , frequent attacks ( usually more than five per day ) ; with marked autonomic features ( rhinorrhoea , nasal congestion , conjunctival injection , lacrimation ) and unilateral to the pain .
	manualset3
120082	10	404840	5	NULL	NULL	0	NULL	lacrimation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Paroxysmal hemicrania has been described as an excruciating unilateral pain , which is usually ocular and frontotemporal with short-lasting ( 2-45 min ) , frequent attacks ( usually more than five per day ) ; with marked autonomic features ( rhinorrhoea , nasal congestion , conjunctival injection , lacrimation ) and unilateral to the pain .
	manualset3
120085	11	404840	5	NULL	NULL	0	NULL	pain 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Paroxysmal hemicrania has been described as an excruciating unilateral pain , which is usually ocular and frontotemporal with short-lasting ( 2-45 min ) , frequent attacks ( usually more than five per day ) ; with marked autonomic features ( rhinorrhoea , nasal congestion , conjunctival injection , lacrimation ) and unilateral to the pain .
	manualset3
120087	1	404841	5	NULL	NULL	0	NULL	introduction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Part 1 : introduction to the International Guidelines 2000 for CPR and ECC .
	manualset3
120088	2	404841	5	NULL	NULL	0	NULL	International Guidelines 2000	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Part 1 : introduction to the International Guidelines 2000 for CPR and ECC .
	manualset3
120092	3	404841	5	NULL	NULL	0	NULL	CPR 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Part 1 : introduction to the International Guidelines 2000 for CPR and ECC .
	manualset3
120093	4	404841	5	NULL	NULL	0	NULL	ECC 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Part 1 : introduction to the International Guidelines 2000 for CPR and ECC .
	manualset3
120097	1	404842	5	NULL	NULL	0	NULL	Postmarketing surveillance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Part I : Postmarketing surveillance within the continuum of the drug approval process .
	manualset3
120098	2	404842	5	NULL	NULL	0	NULL	continuum 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Part I : Postmarketing surveillance within the continuum of the drug approval process .
	manualset3
120099	3	404842	5	NULL	NULL	NULL	NULL	drug approval process	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Part I : Postmarketing surveillance within the continuum of the drug approval process .
	manualset3
120100	1	404843	5	NULL	NULL	0	NULL	Partial correlation analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial correlation analysis controlling for age and sex showed that FSIQ scores were significantly correlated with the FA of the bilateral UF , genu and truncus of CC , bilateral OR and left CST .
	manualset3
120101	2	404843	5	NULL	NULL	0	NULL	age 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial correlation analysis controlling for age and sex showed that FSIQ scores were significantly correlated with the FA of the bilateral UF , genu and truncus of CC , bilateral OR and left CST .
	manualset3
120102	3	404843	5	NULL	NULL	0	NULL	sex 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial correlation analysis controlling for age and sex showed that FSIQ scores were significantly correlated with the FA of the bilateral UF , genu and truncus of CC , bilateral OR and left CST .
	manualset3
120103	4	404843	5	NULL	NULL	0	NULL	FSIQ scores 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial correlation analysis controlling for age and sex showed that FSIQ scores were significantly correlated with the FA of the bilateral UF , genu and truncus of CC , bilateral OR and left CST .
	manualset3
120104	5	404843	5	NULL	NULL	NULL	NULL	FA 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Partial correlation analysis controlling for age and sex showed that FSIQ scores were significantly correlated with the FA of the bilateral UF , genu and truncus of CC , bilateral OR and left CST .
	manualset3
120105	6	404843	5	NULL	NULL	0	NULL	bilateral UF	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial correlation analysis controlling for age and sex showed that FSIQ scores were significantly correlated with the FA of the bilateral UF , genu and truncus of CC , bilateral OR and left CST .
	manualset3
120106	7	404843	5	NULL	NULL	0	NULL	genu of CC	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial correlation analysis controlling for age and sex showed that FSIQ scores were significantly correlated with the FA of the bilateral UF , genu and truncus of CC , bilateral OR and left CST .
	manualset3
120107	8	404843	5	NULL	NULL	0	NULL	truncus of CC	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial correlation analysis controlling for age and sex showed that FSIQ scores were significantly correlated with the FA of the bilateral UF , genu and truncus of CC , bilateral OR and left CST .
	manualset3
120108	9	404843	5	NULL	NULL	0	NULL	bilateral OR	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial correlation analysis controlling for age and sex showed that FSIQ scores were significantly correlated with the FA of the bilateral UF , genu and truncus of CC , bilateral OR and left CST .
	manualset3
120109	10	404843	5	NULL	NULL	0	NULL	left CST	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial correlation analysis controlling for age and sex showed that FSIQ scores were significantly correlated with the FA of the bilateral UF , genu and truncus of CC , bilateral OR and left CST .
	manualset3
120110	1	404844	5	NULL	NULL	0	NULL	Partial deglycosylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial deglycosylation resulted in transformation of the molecule to a more compact state in which phenylalanyl residues were even more buried , tyrosyl residues became more uniform and tryptophyl residues were less exposed .
	manualset3
120111	2	404844	5	NULL	NULL	0	NULL	transformation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial deglycosylation resulted in transformation of the molecule to a more compact state in which phenylalanyl residues were even more buried , tyrosyl residues became more uniform and tryptophyl residues were less exposed .
	manualset3
120112	3	404844	5	NULL	NULL	0	NULL	molecule 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial deglycosylation resulted in transformation of the molecule to a more compact state in which phenylalanyl residues were even more buried , tyrosyl residues became more uniform and tryptophyl residues were less exposed .
	manualset3
120113	4	404844	5	NULL	NULL	0	NULL	compact state	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial deglycosylation resulted in transformation of the molecule to a more compact state in which phenylalanyl residues were even more buried , tyrosyl residues became more uniform and tryptophyl residues were less exposed .
	manualset3
120114	5	404844	5	NULL	NULL	0	NULL	phenylalanyl residues 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial deglycosylation resulted in transformation of the molecule to a more compact state in which phenylalanyl residues were even more buried , tyrosyl residues became more uniform and tryptophyl residues were less exposed .
	manualset3
120115	6	404844	5	NULL	NULL	0	NULL	tyrosyl residues 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial deglycosylation resulted in transformation of the molecule to a more compact state in which phenylalanyl residues were even more buried , tyrosyl residues became more uniform and tryptophyl residues were less exposed .
	manualset3
120116	7	404844	5	NULL	NULL	0	NULL	tryptophyl residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial deglycosylation resulted in transformation of the molecule to a more compact state in which phenylalanyl residues were even more buried , tyrosyl residues became more uniform and tryptophyl residues were less exposed .
	manualset3
120117	1	404845	5	NULL	NULL	0	NULL	Partial liquid ventilation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial liquid ventilation combined with high frequency gas ventilation : clinical breakthrough or two treatments looking for a home ?
	manualset3
120118	2	404845	5	NULL	NULL	0	NULL	high frequency gas ventilation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial liquid ventilation combined with high frequency gas ventilation : clinical breakthrough or two treatments looking for a home ?
	manualset3
120119	3	404845	5	NULL	NULL	0	NULL	clinical breakthrough	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial liquid ventilation combined with high frequency gas ventilation : clinical breakthrough or two treatments looking for a home ?
	manualset3
120124	4	404845	5	NULL	NULL	0	NULL	two treatments	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial liquid ventilation combined with high frequency gas ventilation : clinical breakthrough or two treatments looking for a home ?
	manualset3
120126	5	404845	5	NULL	NULL	0	NULL	home 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial liquid ventilation combined with high frequency gas ventilation : clinical breakthrough or two treatments looking for a home ?
	manualset3
120129	1	404846	5	NULL	NULL	0	NULL	Partial purification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial purification and characterization of the TPI by column chromatography using Sephadex G-150 , papain-Sepharose , and Sephadex G-50 , followed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis , revealed two distinct TPIs with molecular weights of 56 , 000 and 9 , 800 to 10 , 800 .
	manualset3
120131	2	404846	5	NULL	NULL	0	NULL	characterization 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial purification and characterization of the TPI by column chromatography using Sephadex G-150 , papain-Sepharose , and Sephadex G-50 , followed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis , revealed two distinct TPIs with molecular weights of 56 , 000 and 9 , 800 to 10 , 800 .
	manualset3
120132	3	404846	5	NULL	NULL	0	NULL	TPI 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial purification and characterization of the TPI by column chromatography using Sephadex G-150 , papain-Sepharose , and Sephadex G-50 , followed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis , revealed two distinct TPIs with molecular weights of 56 , 000 and 9 , 800 to 10 , 800 .
	manualset3
120133	4	404846	5	NULL	NULL	0	NULL	column chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial purification and characterization of the TPI by column chromatography using Sephadex G-150 , papain-Sepharose , and Sephadex G-50 , followed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis , revealed two distinct TPIs with molecular weights of 56 , 000 and 9 , 800 to 10 , 800 .
	manualset3
120134	5	404846	5	NULL	NULL	0	NULL	Sephadex G-150	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial purification and characterization of the TPI by column chromatography using Sephadex G-150 , papain-Sepharose , and Sephadex G-50 , followed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis , revealed two distinct TPIs with molecular weights of 56 , 000 and 9 , 800 to 10 , 800 .
	manualset3
120135	6	404846	5	NULL	NULL	0	NULL	papain-Sepharose 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial purification and characterization of the TPI by column chromatography using Sephadex G-150 , papain-Sepharose , and Sephadex G-50 , followed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis , revealed two distinct TPIs with molecular weights of 56 , 000 and 9 , 800 to 10 , 800 .
	manualset3
120136	7	404846	5	NULL	NULL	0	NULL	Sephadex G-50 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial purification and characterization of the TPI by column chromatography using Sephadex G-150 , papain-Sepharose , and Sephadex G-50 , followed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis , revealed two distinct TPIs with molecular weights of 56 , 000 and 9 , 800 to 10 , 800 .
	manualset3
120137	8	404846	5	NULL	NULL	0	NULL	sodium dodecyl sulfate-polyacrylamide gel electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial purification and characterization of the TPI by column chromatography using Sephadex G-150 , papain-Sepharose , and Sephadex G-50 , followed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis , revealed two distinct TPIs with molecular weights of 56 , 000 and 9 , 800 to 10 , 800 .
	manualset3
120138	9	404846	5	NULL	NULL	0	NULL	two	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial purification and characterization of the TPI by column chromatography using Sephadex G-150 , papain-Sepharose , and Sephadex G-50 , followed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis , revealed two distinct TPIs with molecular weights of 56 , 000 and 9 , 800 to 10 , 800 .
	manualset3
120139	10	404846	5	NULL	NULL	0	NULL	TPIs 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial purification and characterization of the TPI by column chromatography using Sephadex G-150 , papain-Sepharose , and Sephadex G-50 , followed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis , revealed two distinct TPIs with molecular weights of 56 , 000 and 9 , 800 to 10 , 800 .
	manualset3
120140	11	404846	5	NULL	NULL	0	NULL	molecular weights	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial purification and characterization of the TPI by column chromatography using Sephadex G-150 , papain-Sepharose , and Sephadex G-50 , followed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis , revealed two distinct TPIs with molecular weights of 56 , 000 and 9 , 800 to 10 , 800 .
	manualset3
120141	12	404846	5	NULL	NULL	0	NULL	56 , 000	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial purification and characterization of the TPI by column chromatography using Sephadex G-150 , papain-Sepharose , and Sephadex G-50 , followed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis , revealed two distinct TPIs with molecular weights of 56 , 000 and 9 , 800 to 10 , 800 .
	manualset3
120143	13	404846	5	NULL	NULL	0	NULL	9 , 800 to 10 , 800	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial purification and characterization of the TPI by column chromatography using Sephadex G-150 , papain-Sepharose , and Sephadex G-50 , followed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis , revealed two distinct TPIs with molecular weights of 56 , 000 and 9 , 800 to 10 , 800 .
	manualset3
120147	1	404847	5	NULL	NULL	0	NULL	Partial purification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial purification of membranes and kinetic properties of enzyme .
	manualset3
120149	2	404847	5	NULL	NULL	0	NULL	membranes 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial purification of membranes and kinetic properties of enzyme .
	manualset3
120150	3	404847	5	NULL	NULL	0	NULL	kinetic properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial purification of membranes and kinetic properties of enzyme .
	manualset3
120151	4	404847	5	NULL	NULL	0	NULL	enzyme 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial purification of membranes and kinetic properties of enzyme .
	manualset3
120187	1	404848	5	NULL	NULL	0	NULL	Partial response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial response and stable disease were assessed in 18 % and 56 % of STS patients and in 55 % and 33 % of ABC patients .
	manualset3
120188	2	404848	5	NULL	NULL	0	NULL	stable disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial response and stable disease were assessed in 18 % and 56 % of STS patients and in 55 % and 33 % of ABC patients .
	manualset3
120189	3	404848	5	NULL	NULL	0	NULL	18 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial response and stable disease were assessed in 18 % and 56 % of STS patients and in 55 % and 33 % of ABC patients .
	manualset3
120190	4	404848	5	NULL	NULL	0	NULL	56 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial response and stable disease were assessed in 18 % and 56 % of STS patients and in 55 % and 33 % of ABC patients .
	manualset3
120191	5	404848	5	NULL	NULL	0	NULL	STS patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial response and stable disease were assessed in 18 % and 56 % of STS patients and in 55 % and 33 % of ABC patients .
	manualset3
120193	6	404848	5	NULL	NULL	0	NULL	 55 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial response and stable disease were assessed in 18 % and 56 % of STS patients and in 55 % and 33 % of ABC patients .
	manualset3
120194	7	404848	5	NULL	NULL	0	NULL	33 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial response and stable disease were assessed in 18 % and 56 % of STS patients and in 55 % and 33 % of ABC patients .
	manualset3
120196	8	404848	5	NULL	NULL	0	NULL	ABC patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial response and stable disease were assessed in 18 % and 56 % of STS patients and in 55 % and 33 % of ABC patients .
	manualset3
120213	1	404849	5	NULL	NULL	0	NULL	Participant observation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Participant observation in a suburban high school suggests that adolescents begin smoking as part of a complex symbolic process growing out of the process of social differentiation between future members of the working class on the one hand and the middle class on the other .
	manualset3
120214	2	404849	5	NULL	NULL	0	NULL	suburban high school	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Participant observation in a suburban high school suggests that adolescents begin smoking as part of a complex symbolic process growing out of the process of social differentiation between future members of the working class on the one hand and the middle class on the other .
	manualset3
120215	3	404849	5	NULL	NULL	0	NULL	adolescents 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Participant observation in a suburban high school suggests that adolescents begin smoking as part of a complex symbolic process growing out of the process of social differentiation between future members of the working class on the one hand and the middle class on the other .
	manualset3
120216	4	404849	5	NULL	NULL	0	NULL	smoking 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Participant observation in a suburban high school suggests that adolescents begin smoking as part of a complex symbolic process growing out of the process of social differentiation between future members of the working class on the one hand and the middle class on the other .
	manualset3
120218	5	404849	5	NULL	NULL	0	NULL	complex symbolic process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Participant observation in a suburban high school suggests that adolescents begin smoking as part of a complex symbolic process growing out of the process of social differentiation between future members of the working class on the one hand and the middle class on the other .
	manualset3
120220	6	404849	5	NULL	NULL	0	NULL	process 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Participant observation in a suburban high school suggests that adolescents begin smoking as part of a complex symbolic process growing out of the process of social differentiation between future members of the working class on the one hand and the middle class on the other .
	manualset3
120222	7	404849	5	NULL	NULL	0	NULL	social differentiation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Participant observation in a suburban high school suggests that adolescents begin smoking as part of a complex symbolic process growing out of the process of social differentiation between future members of the working class on the one hand and the middle class on the other .
	manualset3
120223	8	404849	5	NULL	NULL	0	NULL	future members 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Participant observation in a suburban high school suggests that adolescents begin smoking as part of a complex symbolic process growing out of the process of social differentiation between future members of the working class on the one hand and the middle class on the other .
	manualset3
120224	9	404849	5	NULL	NULL	0	NULL	working class	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Participant observation in a suburban high school suggests that adolescents begin smoking as part of a complex symbolic process growing out of the process of social differentiation between future members of the working class on the one hand and the middle class on the other .
	manualset3
120225	10	404849	5	NULL	NULL	0	NULL	one hand	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Participant observation in a suburban high school suggests that adolescents begin smoking as part of a complex symbolic process growing out of the process of social differentiation between future members of the working class on the one hand and the middle class on the other .
	manualset3
120226	11	404849	5	NULL	NULL	0	NULL	middle class	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Participant observation in a suburban high school suggests that adolescents begin smoking as part of a complex symbolic process growing out of the process of social differentiation between future members of the working class on the one hand and the middle class on the other .
	manualset3
120227	1	404850	5	NULL	NULL	0	NULL	60-70 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A further 60-70 % of tumors are of the digestive tract , respiratory tract or urogenital tract .
	manualset3
120228	2	404850	5	NULL	NULL	0	NULL	tumors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A further 60-70 % of tumors are of the digestive tract , respiratory tract or urogenital tract .
	manualset3
120229	3	404850	5	NULL	NULL	0	NULL	digestive tract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A further 60-70 % of tumors are of the digestive tract , respiratory tract or urogenital tract .
	manualset3
120230	4	404850	5	NULL	NULL	0	NULL	respiratory tract 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A further 60-70 % of tumors are of the digestive tract , respiratory tract or urogenital tract .
	manualset3
120231	5	404850	5	NULL	NULL	0	NULL	urogenital tract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A further 60-70 % of tumors are of the digestive tract , respiratory tract or urogenital tract .
	manualset3
120232	1	404851	5	NULL	NULL	0	NULL	Participants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants ' depressive symptoms were assessed via parental reports at the time of the scan and 1 year later .
	manualset3
120233	2	404851	5	NULL	NULL	0	NULL	depressive symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants ' depressive symptoms were assessed via parental reports at the time of the scan and 1 year later .
	manualset3
120234	3	404851	5	NULL	NULL	0	NULL	parental reports	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants ' depressive symptoms were assessed via parental reports at the time of the scan and 1 year later .
	manualset3
120235	4	404851	5	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants ' depressive symptoms were assessed via parental reports at the time of the scan and 1 year later .
	manualset3
120236	5	404851	5	NULL	NULL	0	NULL	scan 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants ' depressive symptoms were assessed via parental reports at the time of the scan and 1 year later .
	manualset3
120237	6	404851	5	NULL	NULL	0	NULL	1 year	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants ' depressive symptoms were assessed via parental reports at the time of the scan and 1 year later .
	manualset3
120238	1	404852	5	NULL	NULL	0	NULL	Participants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants ( n = 148 , mean age 60 years ) had undergone natural menopause and were not using hormone therapy .
	manualset3
120239	2	404852	5	NULL	NULL	0	NULL	 n = 148	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants ( n = 148 , mean age 60 years ) had undergone natural menopause and were not using hormone therapy .
	manualset3
120240	3	404852	5	NULL	NULL	0	NULL	mean age 60 years	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants ( n = 148 , mean age 60 years ) had undergone natural menopause and were not using hormone therapy .
	manualset3
120241	4	404852	5	NULL	NULL	0	NULL	natural menopause 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants ( n = 148 , mean age 60 years ) had undergone natural menopause and were not using hormone therapy .
	manualset3
120242	5	404852	5	NULL	NULL	0	NULL	hormone therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants ( n = 148 , mean age 60 years ) had undergone natural menopause and were not using hormone therapy .
	manualset3
120243	1	404853	5	NULL	NULL	0	NULL	Participants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants also completed a trait empathy scale .
	manualset3
120244	2	404853	5	NULL	NULL	0	NULL	trait empathy scale	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants also completed a trait empathy scale .
	manualset3
120245	1	404854	5	NULL	NULL	0	NULL	Participants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants also indicated satisfaction with the telehealth technology .
	manualset3
120246	2	404854	5	NULL	NULL	0	NULL	satisfaction 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants also indicated satisfaction with the telehealth technology .
	manualset3
120247	3	404854	5	NULL	NULL	0	NULL	telehealth technology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants also indicated satisfaction with the telehealth technology .
	manualset3
120248	1	404855	5	NULL	NULL	0	NULL	Participants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants completed measures of recalled childhood separation anxiety and childhood gender-atypical behavior and identity .
	manualset3
120249	2	404855	5	NULL	NULL	0	NULL	measures 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants completed measures of recalled childhood separation anxiety and childhood gender-atypical behavior and identity .
	manualset3
120251	4	404855	5	NULL	NULL	NULL	NULL	childhood gender-atypical behavior and identity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Participants completed measures of recalled childhood separation anxiety and childhood gender-atypical behavior and identity .
	manualset3
120252	3	404855	5	NULL	NULL	NULL	NULL	childhood separation anxiety	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Participants completed measures of recalled childhood separation anxiety and childhood gender-atypical behavior and identity .
	manualset3
120253	1	404856	5	NULL	NULL	0	NULL	Participants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants in the intervention condition reported more positive gains on measures of self-forgiveness and drinking refusal efficacy , as well as guilt and shame over alcohol-related offenses .
	manualset3
120254	2	404856	5	NULL	NULL	0	NULL	intervention condition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants in the intervention condition reported more positive gains on measures of self-forgiveness and drinking refusal efficacy , as well as guilt and shame over alcohol-related offenses .
	manualset3
120255	3	404856	5	NULL	NULL	0	NULL	positive gains 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants in the intervention condition reported more positive gains on measures of self-forgiveness and drinking refusal efficacy , as well as guilt and shame over alcohol-related offenses .
	manualset3
120256	4	404856	5	NULL	NULL	0	NULL	measures 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants in the intervention condition reported more positive gains on measures of self-forgiveness and drinking refusal efficacy , as well as guilt and shame over alcohol-related offenses .
	manualset3
120257	5	404856	5	NULL	NULL	0	NULL	self-forgiveness	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants in the intervention condition reported more positive gains on measures of self-forgiveness and drinking refusal efficacy , as well as guilt and shame over alcohol-related offenses .
	manualset3
120258	6	404856	5	NULL	NULL	0	NULL	drinking refusal efficacy	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants in the intervention condition reported more positive gains on measures of self-forgiveness and drinking refusal efficacy , as well as guilt and shame over alcohol-related offenses .
	manualset3
120259	7	404856	5	NULL	NULL	0	NULL	guilt 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants in the intervention condition reported more positive gains on measures of self-forgiveness and drinking refusal efficacy , as well as guilt and shame over alcohol-related offenses .
	manualset3
120260	8	404856	5	NULL	NULL	0	NULL	shame 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants in the intervention condition reported more positive gains on measures of self-forgiveness and drinking refusal efficacy , as well as guilt and shame over alcohol-related offenses .
	manualset3
120261	9	404856	5	NULL	NULL	0	NULL	alcohol-related offenses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants in the intervention condition reported more positive gains on measures of self-forgiveness and drinking refusal efficacy , as well as guilt and shame over alcohol-related offenses .
	manualset3
120315	1	404857	5	NULL	NULL	0	NULL	Participants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants learned a complex video game for 30h ( Space Fortress , Donchin , Fabiani , & Sanders , 1989 ) using one of two training regimens : Hybrid Variable-Priority Training ( HVT ) , with a focus on improving specific skills and managing task priority , or Full Emphasis Training ( FET ) in which participants simply practiced the game to obtain the highest overall score .
	manualset3
120316	2	404857	5	NULL	NULL	0	NULL	complex video game	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants learned a complex video game for 30h ( Space Fortress , Donchin , Fabiani , & Sanders , 1989 ) using one of two training regimens : Hybrid Variable-Priority Training ( HVT ) , with a focus on improving specific skills and managing task priority , or Full Emphasis Training ( FET ) in which participants simply practiced the game to obtain the highest overall score .
	manualset3
120317	3	404857	5	NULL	NULL	0	NULL	 30h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants learned a complex video game for 30h ( Space Fortress , Donchin , Fabiani , & Sanders , 1989 ) using one of two training regimens : Hybrid Variable-Priority Training ( HVT ) , with a focus on improving specific skills and managing task priority , or Full Emphasis Training ( FET ) in which participants simply practiced the game to obtain the highest overall score .
	manualset3
120318	4	404857	5	NULL	NULL	0	NULL	Space Fortress , Donchin , Fabiani , & Sanders , 1989	Citation												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants learned a complex video game for 30h ( Space Fortress , Donchin , Fabiani , & Sanders , 1989 ) using one of two training regimens : Hybrid Variable-Priority Training ( HVT ) , with a focus on improving specific skills and managing task priority , or Full Emphasis Training ( FET ) in which participants simply practiced the game to obtain the highest overall score .
	manualset3
120319	5	404857	5	NULL	NULL	0	NULL	one 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants learned a complex video game for 30h ( Space Fortress , Donchin , Fabiani , & Sanders , 1989 ) using one of two training regimens : Hybrid Variable-Priority Training ( HVT ) , with a focus on improving specific skills and managing task priority , or Full Emphasis Training ( FET ) in which participants simply practiced the game to obtain the highest overall score .
	manualset3
120320	6	404857	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants learned a complex video game for 30h ( Space Fortress , Donchin , Fabiani , & Sanders , 1989 ) using one of two training regimens : Hybrid Variable-Priority Training ( HVT ) , with a focus on improving specific skills and managing task priority , or Full Emphasis Training ( FET ) in which participants simply practiced the game to obtain the highest overall score .
	manualset3
120321	7	404857	5	NULL	NULL	0	NULL	training regimens	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants learned a complex video game for 30h ( Space Fortress , Donchin , Fabiani , & Sanders , 1989 ) using one of two training regimens : Hybrid Variable-Priority Training ( HVT ) , with a focus on improving specific skills and managing task priority , or Full Emphasis Training ( FET ) in which participants simply practiced the game to obtain the highest overall score .
	manualset3
120322	8	404857	5	NULL	NULL	0	NULL	Hybrid Variable-Priority Training ( HVT ) 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants learned a complex video game for 30h ( Space Fortress , Donchin , Fabiani , & Sanders , 1989 ) using one of two training regimens : Hybrid Variable-Priority Training ( HVT ) , with a focus on improving specific skills and managing task priority , or Full Emphasis Training ( FET ) in which participants simply practiced the game to obtain the highest overall score .
	manualset3
120323	9	404857	5	NULL	NULL	0	NULL	focus 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants learned a complex video game for 30h ( Space Fortress , Donchin , Fabiani , & Sanders , 1989 ) using one of two training regimens : Hybrid Variable-Priority Training ( HVT ) , with a focus on improving specific skills and managing task priority , or Full Emphasis Training ( FET ) in which participants simply practiced the game to obtain the highest overall score .
	manualset3
120324	10	404857	5	NULL	NULL	0	NULL	specific skills	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants learned a complex video game for 30h ( Space Fortress , Donchin , Fabiani , & Sanders , 1989 ) using one of two training regimens : Hybrid Variable-Priority Training ( HVT ) , with a focus on improving specific skills and managing task priority , or Full Emphasis Training ( FET ) in which participants simply practiced the game to obtain the highest overall score .
	manualset3
120325	11	404857	5	NULL	NULL	0	NULL	task priority	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants learned a complex video game for 30h ( Space Fortress , Donchin , Fabiani , & Sanders , 1989 ) using one of two training regimens : Hybrid Variable-Priority Training ( HVT ) , with a focus on improving specific skills and managing task priority , or Full Emphasis Training ( FET ) in which participants simply practiced the game to obtain the highest overall score .
	manualset3
120326	12	404857	5	NULL	NULL	0	NULL	Full Emphasis Training ( FET )	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants learned a complex video game for 30h ( Space Fortress , Donchin , Fabiani , & Sanders , 1989 ) using one of two training regimens : Hybrid Variable-Priority Training ( HVT ) , with a focus on improving specific skills and managing task priority , or Full Emphasis Training ( FET ) in which participants simply practiced the game to obtain the highest overall score .
	manualset3
120327	13	404857	5	NULL	NULL	0	NULL	participants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants learned a complex video game for 30h ( Space Fortress , Donchin , Fabiani , & Sanders , 1989 ) using one of two training regimens : Hybrid Variable-Priority Training ( HVT ) , with a focus on improving specific skills and managing task priority , or Full Emphasis Training ( FET ) in which participants simply practiced the game to obtain the highest overall score .
	manualset3
120328	14	404857	5	NULL	NULL	0	NULL	game 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants learned a complex video game for 30h ( Space Fortress , Donchin , Fabiani , & Sanders , 1989 ) using one of two training regimens : Hybrid Variable-Priority Training ( HVT ) , with a focus on improving specific skills and managing task priority , or Full Emphasis Training ( FET ) in which participants simply practiced the game to obtain the highest overall score .
	manualset3
120329	15	404857	5	NULL	NULL	0	NULL	highest overall score	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants learned a complex video game for 30h ( Space Fortress , Donchin , Fabiani , & Sanders , 1989 ) using one of two training regimens : Hybrid Variable-Priority Training ( HVT ) , with a focus on improving specific skills and managing task priority , or Full Emphasis Training ( FET ) in which participants simply practiced the game to obtain the highest overall score .
	manualset3
120330	1	404858	5	NULL	NULL	0	NULL	Participants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants read aloud third , sixth , and ninth grade level material in non-altered auditory feedback ( NAF ) and FAF conditions .
	manualset3
120331	2	404858	5	NULL	NULL	NULL	NULL	read aloud	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Participants read aloud third , sixth , and ninth grade level material in non-altered auditory feedback ( NAF ) and FAF conditions .
	manualset3
120498	3	404858	5	NULL	NULL	0	NULL	third grade level material	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants read aloud third , sixth , and ninth grade level material in non-altered auditory feedback ( NAF ) and FAF conditions .
	manualset3
120499	4	404858	5	NULL	NULL	0	NULL	sixth grade level material	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants read aloud third , sixth , and ninth grade level material in non-altered auditory feedback ( NAF ) and FAF conditions .
	manualset3
120500	5	404858	5	NULL	NULL	0	NULL	ninth grade level material	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants read aloud third , sixth , and ninth grade level material in non-altered auditory feedback ( NAF ) and FAF conditions .
	manualset3
120501	6	404858	5	NULL	NULL	0	NULL	non-altered auditory feedback ( NAF )	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants read aloud third , sixth , and ninth grade level material in non-altered auditory feedback ( NAF ) and FAF conditions .
	manualset3
120502	7	404858	5	NULL	NULL	0	NULL	 FAF conditions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants read aloud third , sixth , and ninth grade level material in non-altered auditory feedback ( NAF ) and FAF conditions .
	manualset3
120503	1	404859	5	NULL	NULL	0	NULL	Participants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants supplemented their daily diets with 42 g of margarine spread ( PSE = 3 g ; CON , PSE = 0 g , of approximately equal energy content ) for 9 weeks .
	manualset3
120504	2	404859	5	NULL	NULL	0	NULL	daily diets	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants supplemented their daily diets with 42 g of margarine spread ( PSE = 3 g ; CON , PSE = 0 g , of approximately equal energy content ) for 9 weeks .
	manualset3
120505	3	404859	5	NULL	NULL	0	NULL	42 g	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants supplemented their daily diets with 42 g of margarine spread ( PSE = 3 g ; CON , PSE = 0 g , of approximately equal energy content ) for 9 weeks .
	manualset3
120506	4	404859	5	NULL	NULL	0	NULL	margarine spread	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants supplemented their daily diets with 42 g of margarine spread ( PSE = 3 g ; CON , PSE = 0 g , of approximately equal energy content ) for 9 weeks .
	manualset3
120507	5	404859	5	NULL	NULL	0	NULL	PSE = 3 g	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants supplemented their daily diets with 42 g of margarine spread ( PSE = 3 g ; CON , PSE = 0 g , of approximately equal energy content ) for 9 weeks .
	manualset3
120508	6	404859	5	NULL	NULL	0	NULL	CON , PSE = 0 g	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants supplemented their daily diets with 42 g of margarine spread ( PSE = 3 g ; CON , PSE = 0 g , of approximately equal energy content ) for 9 weeks .
	manualset3
120509	7	404859	5	NULL	NULL	0	NULL	energy content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants supplemented their daily diets with 42 g of margarine spread ( PSE = 3 g ; CON , PSE = 0 g , of approximately equal energy content ) for 9 weeks .
	manualset3
120510	8	404859	5	NULL	NULL	0	NULL	9 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants supplemented their daily diets with 42 g of margarine spread ( PSE = 3 g ; CON , PSE = 0 g , of approximately equal energy content ) for 9 weeks .
	manualset3
120511	1	404860	5	NULL	NULL	0	NULL	Participants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants using the CF ranked the quality of the article without the assistance of the quality assessment form .
	manualset3
120512	2	404860	5	NULL	NULL	0	NULL	CF 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants using the CF ranked the quality of the article without the assistance of the quality assessment form .
	manualset3
120513	3	404860	5	NULL	NULL	0	NULL	quality 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants using the CF ranked the quality of the article without the assistance of the quality assessment form .
	manualset3
120514	4	404860	5	NULL	NULL	0	NULL	article 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants using the CF ranked the quality of the article without the assistance of the quality assessment form .
	manualset3
120515	5	404860	5	NULL	NULL	0	NULL	assistance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants using the CF ranked the quality of the article without the assistance of the quality assessment form .
	manualset3
120516	6	404860	5	NULL	NULL	0	NULL	quality assessment form	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants using the CF ranked the quality of the article without the assistance of the quality assessment form .
	manualset3
120517	1	404861	5	NULL	NULL	0	NULL	Participants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants were categorized according to whether their terminal degree was a bachelor 's , master 's , or doctorate degree , and within these degree groupings , the proportion of participants with at least one patent or scientific publication in adulthood increased as a function of this early SAT assessment .
	manualset3
120518	2	404861	5	NULL	NULL	0	NULL	terminal degree 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants were categorized according to whether their terminal degree was a bachelor 's , master 's , or doctorate degree , and within these degree groupings , the proportion of participants with at least one patent or scientific publication in adulthood increased as a function of this early SAT assessment .
	manualset3
120519	3	404861	5	NULL	NULL	0	NULL	bachelor 's degree	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants were categorized according to whether their terminal degree was a bachelor 's , master 's , or doctorate degree , and within these degree groupings , the proportion of participants with at least one patent or scientific publication in adulthood increased as a function of this early SAT assessment .
	manualset3
120520	4	404861	5	NULL	NULL	0	NULL	master 's degree	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants were categorized according to whether their terminal degree was a bachelor 's , master 's , or doctorate degree , and within these degree groupings , the proportion of participants with at least one patent or scientific publication in adulthood increased as a function of this early SAT assessment .
	manualset3
120521	5	404861	5	NULL	NULL	0	NULL	doctorate degree	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants were categorized according to whether their terminal degree was a bachelor 's , master 's , or doctorate degree , and within these degree groupings , the proportion of participants with at least one patent or scientific publication in adulthood increased as a function of this early SAT assessment .
	manualset3
120522	6	404861	5	NULL	NULL	0	NULL	degree groupings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants were categorized according to whether their terminal degree was a bachelor 's , master 's , or doctorate degree , and within these degree groupings , the proportion of participants with at least one patent or scientific publication in adulthood increased as a function of this early SAT assessment .
	manualset3
120523	7	404861	5	NULL	NULL	0	NULL	proportion 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants were categorized according to whether their terminal degree was a bachelor 's , master 's , or doctorate degree , and within these degree groupings , the proportion of participants with at least one patent or scientific publication in adulthood increased as a function of this early SAT assessment .
	manualset3
120524	8	404861	5	NULL	NULL	0	NULL	participants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants were categorized according to whether their terminal degree was a bachelor 's , master 's , or doctorate degree , and within these degree groupings , the proportion of participants with at least one patent or scientific publication in adulthood increased as a function of this early SAT assessment .
	manualset3
120525	9	404861	5	NULL	NULL	0	NULL	one 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants were categorized according to whether their terminal degree was a bachelor 's , master 's , or doctorate degree , and within these degree groupings , the proportion of participants with at least one patent or scientific publication in adulthood increased as a function of this early SAT assessment .
	manualset3
120526	10	404861	5	NULL	NULL	0	NULL	patent 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants were categorized according to whether their terminal degree was a bachelor 's , master 's , or doctorate degree , and within these degree groupings , the proportion of participants with at least one patent or scientific publication in adulthood increased as a function of this early SAT assessment .
	manualset3
120527	11	404861	5	NULL	NULL	0	NULL	scientific publication	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants were categorized according to whether their terminal degree was a bachelor 's , master 's , or doctorate degree , and within these degree groupings , the proportion of participants with at least one patent or scientific publication in adulthood increased as a function of this early SAT assessment .
	manualset3
120528	12	404861	5	NULL	NULL	0	NULL	adulthood 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants were categorized according to whether their terminal degree was a bachelor 's , master 's , or doctorate degree , and within these degree groupings , the proportion of participants with at least one patent or scientific publication in adulthood increased as a function of this early SAT assessment .
	manualset3
120529	13	404861	5	NULL	NULL	0	NULL	function 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants were categorized according to whether their terminal degree was a bachelor 's , master 's , or doctorate degree , and within these degree groupings , the proportion of participants with at least one patent or scientific publication in adulthood increased as a function of this early SAT assessment .
	manualset3
120530	14	404861	5	NULL	NULL	0	NULL	early SAT assessment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants were categorized according to whether their terminal degree was a bachelor 's , master 's , or doctorate degree , and within these degree groupings , the proportion of participants with at least one patent or scientific publication in adulthood increased as a function of this early SAT assessment .
	manualset3
120531	1	404862	5	NULL	NULL	0	NULL	Participants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants were more certain that the stimulus described a rape , recommended a longer prison sentence for the offender , and assigned less blame to the victim when exposed to an offender motivated by violence as opposed to an offender motivated by sex .
	manualset3
120532	2	404862	5	NULL	NULL	0	NULL	stimulus 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants were more certain that the stimulus described a rape , recommended a longer prison sentence for the offender , and assigned less blame to the victim when exposed to an offender motivated by violence as opposed to an offender motivated by sex .
	manualset3
120533	3	404862	5	NULL	NULL	0	NULL	rape 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants were more certain that the stimulus described a rape , recommended a longer prison sentence for the offender , and assigned less blame to the victim when exposed to an offender motivated by violence as opposed to an offender motivated by sex .
	manualset3
120534	4	404862	5	NULL	NULL	0	NULL	longer prison sentence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants were more certain that the stimulus described a rape , recommended a longer prison sentence for the offender , and assigned less blame to the victim when exposed to an offender motivated by violence as opposed to an offender motivated by sex .
	manualset3
120535	5	404862	5	NULL	NULL	0	NULL	offender 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants were more certain that the stimulus described a rape , recommended a longer prison sentence for the offender , and assigned less blame to the victim when exposed to an offender motivated by violence as opposed to an offender motivated by sex .
	manualset3
120536	6	404862	5	NULL	NULL	0	NULL	blame 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants were more certain that the stimulus described a rape , recommended a longer prison sentence for the offender , and assigned less blame to the victim when exposed to an offender motivated by violence as opposed to an offender motivated by sex .
	manualset3
120537	7	404862	5	NULL	NULL	0	NULL	victim 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants were more certain that the stimulus described a rape , recommended a longer prison sentence for the offender , and assigned less blame to the victim when exposed to an offender motivated by violence as opposed to an offender motivated by sex .
	manualset3
120538	8	404862	5	NULL	NULL	0	NULL	offender 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants were more certain that the stimulus described a rape , recommended a longer prison sentence for the offender , and assigned less blame to the victim when exposed to an offender motivated by violence as opposed to an offender motivated by sex .
	manualset3
120539	9	404862	5	NULL	NULL	0	NULL	violence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants were more certain that the stimulus described a rape , recommended a longer prison sentence for the offender , and assigned less blame to the victim when exposed to an offender motivated by violence as opposed to an offender motivated by sex .
	manualset3
120540	10	404862	5	NULL	NULL	0	NULL	offender 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants were more certain that the stimulus described a rape , recommended a longer prison sentence for the offender , and assigned less blame to the victim when exposed to an offender motivated by violence as opposed to an offender motivated by sex .
	manualset3
120541	11	404862	5	NULL	NULL	0	NULL	sex 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants were more certain that the stimulus described a rape , recommended a longer prison sentence for the offender , and assigned less blame to the victim when exposed to an offender motivated by violence as opposed to an offender motivated by sex .
	manualset3
120542	1	404863	5	NULL	NULL	0	NULL	Participants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants with a family history of breast cancer were significantly more likely to know that genes had been identified that indicate an increased risk of breast cancer ( p & lt ; 0.05 ) .
	manualset3
120543	2	404863	5	NULL	NULL	NULL	NULL	family history	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Participants with a family history of breast cancer were significantly more likely to know that genes had been identified that indicate an increased risk of breast cancer ( p & lt ; 0.05 ) .
	manualset3
120544	3	404863	5	NULL	NULL	0	NULL	breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants with a family history of breast cancer were significantly more likely to know that genes had been identified that indicate an increased risk of breast cancer ( p & lt ; 0.05 ) .
	manualset3
120545	4	404863	5	NULL	NULL	0	NULL	genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants with a family history of breast cancer were significantly more likely to know that genes had been identified that indicate an increased risk of breast cancer ( p & lt ; 0.05 ) .
	manualset3
120546	5	404863	5	NULL	NULL	0	NULL	increased risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants with a family history of breast cancer were significantly more likely to know that genes had been identified that indicate an increased risk of breast cancer ( p & lt ; 0.05 ) .
	manualset3
120547	6	404863	5	NULL	NULL	0	NULL	breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants with a family history of breast cancer were significantly more likely to know that genes had been identified that indicate an increased risk of breast cancer ( p & lt ; 0.05 ) .
	manualset3
120548	7	404863	5	NULL	NULL	0	NULL	p & lt ; 0.05 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Participants with a family history of breast cancer were significantly more likely to know that genes had been identified that indicate an increased risk of breast cancer ( p & lt ; 0.05 ) .
	manualset3
120549	1	404864	5	NULL	NULL	0	NULL	Particle deposition measurements 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Particle deposition measurements were conducted by gravimetry .
	manualset3
120550	2	404864	5	NULL	NULL	0	NULL	gravimetry 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Particle deposition measurements were conducted by gravimetry .
	manualset3
120551	1	404865	5	NULL	NULL	0	NULL	Particle surface geometry	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Particle surface geometry was found to influence precursor dissolution , with planar particles stabilizing the shear-induced precursors to a much greater extent than curved particles .
	manualset3
120552	2	404865	5	NULL	NULL	0	NULL	precursor dissolution 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Particle surface geometry was found to influence precursor dissolution , with planar particles stabilizing the shear-induced precursors to a much greater extent than curved particles .
	manualset3
120553	3	404865	5	NULL	NULL	0	NULL	planar particles 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Particle surface geometry was found to influence precursor dissolution , with planar particles stabilizing the shear-induced precursors to a much greater extent than curved particles .
	manualset3
120554	4	404865	5	NULL	NULL	0	NULL	shear-induced precursors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Particle surface geometry was found to influence precursor dissolution , with planar particles stabilizing the shear-induced precursors to a much greater extent than curved particles .
	manualset3
120555	5	404865	5	NULL	NULL	0	NULL	greater extent 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Particle surface geometry was found to influence precursor dissolution , with planar particles stabilizing the shear-induced precursors to a much greater extent than curved particles .
	manualset3
120556	6	404865	5	NULL	NULL	0	NULL	curved particles	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Particle surface geometry was found to influence precursor dissolution , with planar particles stabilizing the shear-induced precursors to a much greater extent than curved particles .
	manualset3
120557	1	404866	5	NULL	NULL	0	NULL	fusion protein	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A fusion protein containing either full-length A20R or only the N-terminal 25 amino acids of A20R was sufficient to capture the D4R protein , whereas the fusion protein containing A20R amino acids 26 to 426 was not , confirming the results of the yeast two-hybrid analysis .
	manualset3
120558	2	404866	5	NULL	NULL	0	NULL	full-length A20R	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A fusion protein containing either full-length A20R or only the N-terminal 25 amino acids of A20R was sufficient to capture the D4R protein , whereas the fusion protein containing A20R amino acids 26 to 426 was not , confirming the results of the yeast two-hybrid analysis .
	manualset3
120559	3	404866	5	NULL	NULL	0	NULL	N-terminal 25 amino acids of A20R 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A fusion protein containing either full-length A20R or only the N-terminal 25 amino acids of A20R was sufficient to capture the D4R protein , whereas the fusion protein containing A20R amino acids 26 to 426 was not , confirming the results of the yeast two-hybrid analysis .
	manualset3
120560	4	404866	5	NULL	NULL	0	NULL	D4R protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A fusion protein containing either full-length A20R or only the N-terminal 25 amino acids of A20R was sufficient to capture the D4R protein , whereas the fusion protein containing A20R amino acids 26 to 426 was not , confirming the results of the yeast two-hybrid analysis .
	manualset3
120561	5	404866	5	NULL	NULL	NULL	NULL	fusion protein	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A fusion protein containing either full-length A20R or only the N-terminal 25 amino acids of A20R was sufficient to capture the D4R protein , whereas the fusion protein containing A20R amino acids 26 to 426 was not , confirming the results of the yeast two-hybrid analysis .
	manualset3
120562	6	404866	5	NULL	NULL	0	NULL	A20R amino acids 26 to 426 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A fusion protein containing either full-length A20R or only the N-terminal 25 amino acids of A20R was sufficient to capture the D4R protein , whereas the fusion protein containing A20R amino acids 26 to 426 was not , confirming the results of the yeast two-hybrid analysis .
	manualset3
120563	7	404866	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A fusion protein containing either full-length A20R or only the N-terminal 25 amino acids of A20R was sufficient to capture the D4R protein , whereas the fusion protein containing A20R amino acids 26 to 426 was not , confirming the results of the yeast two-hybrid analysis .
	manualset3
120564	8	404866	5	NULL	NULL	0	NULL	yeast two-hybrid analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A fusion protein containing either full-length A20R or only the N-terminal 25 amino acids of A20R was sufficient to capture the D4R protein , whereas the fusion protein containing A20R amino acids 26 to 426 was not , confirming the results of the yeast two-hybrid analysis .
	manualset3
120565	1	404867	5	NULL	NULL	0	NULL	attention	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Particular attention is drawn to the morphological changes in the curve .
	manualset3
120566	2	404867	5	NULL	NULL	0	NULL	morphological changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Particular attention is drawn to the morphological changes in the curve .
	manualset3
120567	3	404867	5	NULL	NULL	0	NULL	curve	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Particular attention is drawn to the morphological changes in the curve .
	manualset3
120568	1	404868	5	NULL	NULL	0	NULL	effort	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Particular effort has been devoted to developing a sample-processing technique that allows the total amount of tellurium and isotope ratios to be measured by graphite furnace atomic absorption spectrometry ( GFAAS ) and secondary ion mass spectrometry ( SIMS ) , respectively .
	manualset3
120569	2	404868	5	NULL	NULL	0	NULL	sample-processing technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Particular effort has been devoted to developing a sample-processing technique that allows the total amount of tellurium and isotope ratios to be measured by graphite furnace atomic absorption spectrometry ( GFAAS ) and secondary ion mass spectrometry ( SIMS ) , respectively .
	manualset3
120570	3	404868	5	NULL	NULL	0	NULL	total amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Particular effort has been devoted to developing a sample-processing technique that allows the total amount of tellurium and isotope ratios to be measured by graphite furnace atomic absorption spectrometry ( GFAAS ) and secondary ion mass spectrometry ( SIMS ) , respectively .
	manualset3
120571	4	404868	5	NULL	NULL	0	NULL	tellurium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Particular effort has been devoted to developing a sample-processing technique that allows the total amount of tellurium and isotope ratios to be measured by graphite furnace atomic absorption spectrometry ( GFAAS ) and secondary ion mass spectrometry ( SIMS ) , respectively .
	manualset3
120572	5	404868	5	NULL	NULL	0	NULL	isotope ratios	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Particular effort has been devoted to developing a sample-processing technique that allows the total amount of tellurium and isotope ratios to be measured by graphite furnace atomic absorption spectrometry ( GFAAS ) and secondary ion mass spectrometry ( SIMS ) , respectively .
	manualset3
120573	6	404868	5	NULL	NULL	0	NULL	graphite furnace atomic absorption spectrometry ( GFAAS )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Particular effort has been devoted to developing a sample-processing technique that allows the total amount of tellurium and isotope ratios to be measured by graphite furnace atomic absorption spectrometry ( GFAAS ) and secondary ion mass spectrometry ( SIMS ) , respectively .
	manualset3
120574	7	404868	5	NULL	NULL	0	NULL	secondary ion mass spectrometry ( SIMS )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Particular effort has been devoted to developing a sample-processing technique that allows the total amount of tellurium and isotope ratios to be measured by graphite furnace atomic absorption spectrometry ( GFAAS ) and secondary ion mass spectrometry ( SIMS ) , respectively .
	manualset3
120575	1	404869	5	NULL	NULL	0	NULL	emphasis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Particular emphasis is placed on learning from developing country experience .
	manualset3
120576	2	404869	5	NULL	NULL	0	NULL	learning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Particular emphasis is placed on learning from developing country experience .
	manualset3
120577	3	404869	5	NULL	NULL	0	NULL	developing country experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Particular emphasis is placed on learning from developing country experience .
	manualset3
120578	1	404870	5	NULL	NULL	0	NULL	emphasis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Particular emphasis was placed on the importance of incorporating the interreplication variance in statistical models and estimating confidence intervals .
	manualset3
120579	2	404870	5	NULL	NULL	0	NULL	importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Particular emphasis was placed on the importance of incorporating the interreplication variance in statistical models and estimating confidence intervals .
	manualset3
120580	3	404870	5	NULL	NULL	NULL	NULL	interreplication variance	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Particular emphasis was placed on the importance of incorporating the interreplication variance in statistical models and estimating confidence intervals .
	manualset3
120581	4	404870	5	NULL	NULL	0	NULL	statistical models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Particular emphasis was placed on the importance of incorporating the interreplication variance in statistical models and estimating confidence intervals .
	manualset3
120582	5	404870	5	NULL	NULL	0	NULL	confidence intervals	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Particular emphasis was placed on the importance of incorporating the interreplication variance in statistical models and estimating confidence intervals .
	manualset3
120583	1	404871	5	NULL	NULL	0	NULL	microbial characteristics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Particular microbial characteristics as well as the type of the inflammatory response contribute to clinical outcomes via influence on epithelial cell and immune responses .
	manualset3
120584	2	404871	5	NULL	NULL	0	NULL	type	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Particular microbial characteristics as well as the type of the inflammatory response contribute to clinical outcomes via influence on epithelial cell and immune responses .
	manualset3
120585	3	404871	5	NULL	NULL	0	NULL	inflammatory response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Particular microbial characteristics as well as the type of the inflammatory response contribute to clinical outcomes via influence on epithelial cell and immune responses .
	manualset3
120586	4	404871	5	NULL	NULL	0	NULL	clinical outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Particular microbial characteristics as well as the type of the inflammatory response contribute to clinical outcomes via influence on epithelial cell and immune responses .
	manualset3
120587	5	404871	5	NULL	NULL	0	NULL	influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Particular microbial characteristics as well as the type of the inflammatory response contribute to clinical outcomes via influence on epithelial cell and immune responses .
	manualset3
120588	6	404871	5	NULL	NULL	0	NULL	epithelial cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Particular microbial characteristics as well as the type of the inflammatory response contribute to clinical outcomes via influence on epithelial cell and immune responses .
	manualset3
120589	7	404871	5	NULL	NULL	0	NULL	immune responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Particular microbial characteristics as well as the type of the inflammatory response contribute to clinical outcomes via influence on epithelial cell and immune responses .
	manualset3
120590	1	404872	5	NULL	NULL	0	NULL	PE intensities 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly , the PE intensities of the f-derived bands are correctly reproduced for photon energies between 60 and 103 eV .
	manualset3
120591	2	404872	5	NULL	NULL	0	NULL	f-derived bands	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly , the PE intensities of the f-derived bands are correctly reproduced for photon energies between 60 and 103 eV .
	manualset3
120592	3	404872	5	NULL	NULL	0	NULL	photon energies	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly , the PE intensities of the f-derived bands are correctly reproduced for photon energies between 60 and 103 eV .
	manualset3
120593	4	404872	5	NULL	NULL	NULL	NULL	60 eV	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Particularly , the PE intensities of the f-derived bands are correctly reproduced for photon energies between 60 and 103 eV .
	manualset3
120594	5	404872	5	NULL	NULL	0	NULL	103 eV	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly , the PE intensities of the f-derived bands are correctly reproduced for photon energies between 60 and 103 eV .
	manualset3
120595	1	404873	5	NULL	NULL	0	NULL	galI-disruption mutant ( SK-galI-5 )	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A galI-disruption mutant ( SK-galI-5 ) is unable to produce galbonolide A , but can synthesize galbonolide B , indicating that galGHIJK is involved in the biosynthesis of galbonolide A. A disruption mutant of orf4 is severely impaired in the production of both galbonolides A and B. These results indicate that galGHIJK and the KAS genes are involved in the biosynthesis of galbonolides , although they are not colocalized with a multimodular PKS gene cluster .
	manualset3
120596	2	404873	5	NULL	NULL	0	NULL	galbonolide A	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A galI-disruption mutant ( SK-galI-5 ) is unable to produce galbonolide A , but can synthesize galbonolide B , indicating that galGHIJK is involved in the biosynthesis of galbonolide A. A disruption mutant of orf4 is severely impaired in the production of both galbonolides A and B. These results indicate that galGHIJK and the KAS genes are involved in the biosynthesis of galbonolides , although they are not colocalized with a multimodular PKS gene cluster .
	manualset3
120597	3	404873	5	NULL	NULL	0	NULL	galbonolide B	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A galI-disruption mutant ( SK-galI-5 ) is unable to produce galbonolide A , but can synthesize galbonolide B , indicating that galGHIJK is involved in the biosynthesis of galbonolide A. A disruption mutant of orf4 is severely impaired in the production of both galbonolides A and B. These results indicate that galGHIJK and the KAS genes are involved in the biosynthesis of galbonolides , although they are not colocalized with a multimodular PKS gene cluster .
	manualset3
120598	4	404873	5	NULL	NULL	NULL	NULL	galGHIJK	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A galI-disruption mutant ( SK-galI-5 ) is unable to produce galbonolide A , but can synthesize galbonolide B , indicating that galGHIJK is involved in the biosynthesis of galbonolide A. A disruption mutant of orf4 is severely impaired in the production of both galbonolides A and B. These results indicate that galGHIJK and the KAS genes are involved in the biosynthesis of galbonolides , although they are not colocalized with a multimodular PKS gene cluster .
	manualset3
120599	5	404873	5	NULL	NULL	0	NULL	biosynthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A galI-disruption mutant ( SK-galI-5 ) is unable to produce galbonolide A , but can synthesize galbonolide B , indicating that galGHIJK is involved in the biosynthesis of galbonolide A. A disruption mutant of orf4 is severely impaired in the production of both galbonolides A and B. These results indicate that galGHIJK and the KAS genes are involved in the biosynthesis of galbonolides , although they are not colocalized with a multimodular PKS gene cluster .
	manualset3
120600	6	404873	5	NULL	NULL	0	NULL	galbonolide A	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A galI-disruption mutant ( SK-galI-5 ) is unable to produce galbonolide A , but can synthesize galbonolide B , indicating that galGHIJK is involved in the biosynthesis of galbonolide A. A disruption mutant of orf4 is severely impaired in the production of both galbonolides A and B. These results indicate that galGHIJK and the KAS genes are involved in the biosynthesis of galbonolides , although they are not colocalized with a multimodular PKS gene cluster .
	manualset3
120601	7	404873	5	NULL	NULL	0	NULL	disruption mutant	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A galI-disruption mutant ( SK-galI-5 ) is unable to produce galbonolide A , but can synthesize galbonolide B , indicating that galGHIJK is involved in the biosynthesis of galbonolide A. A disruption mutant of orf4 is severely impaired in the production of both galbonolides A and B. These results indicate that galGHIJK and the KAS genes are involved in the biosynthesis of galbonolides , although they are not colocalized with a multimodular PKS gene cluster .
	manualset3
120602	8	404873	5	NULL	NULL	NULL	NULL	orf4	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A galI-disruption mutant ( SK-galI-5 ) is unable to produce galbonolide A , but can synthesize galbonolide B , indicating that galGHIJK is involved in the biosynthesis of galbonolide A. A disruption mutant of orf4 is severely impaired in the production of both galbonolides A and B. These results indicate that galGHIJK and the KAS genes are involved in the biosynthesis of galbonolides , although they are not colocalized with a multimodular PKS gene cluster .
	manualset3
120603	9	404873	5	NULL	NULL	0	NULL	production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A galI-disruption mutant ( SK-galI-5 ) is unable to produce galbonolide A , but can synthesize galbonolide B , indicating that galGHIJK is involved in the biosynthesis of galbonolide A. A disruption mutant of orf4 is severely impaired in the production of both galbonolides A and B. These results indicate that galGHIJK and the KAS genes are involved in the biosynthesis of galbonolides , although they are not colocalized with a multimodular PKS gene cluster .
	manualset3
120604	10	404873	5	NULL	NULL	0	NULL	galbonolides A	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A galI-disruption mutant ( SK-galI-5 ) is unable to produce galbonolide A , but can synthesize galbonolide B , indicating that galGHIJK is involved in the biosynthesis of galbonolide A. A disruption mutant of orf4 is severely impaired in the production of both galbonolides A and B. These results indicate that galGHIJK and the KAS genes are involved in the biosynthesis of galbonolides , although they are not colocalized with a multimodular PKS gene cluster .
	manualset3
120605	11	404873	5	NULL	NULL	0	NULL	galbonolides B	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A galI-disruption mutant ( SK-galI-5 ) is unable to produce galbonolide A , but can synthesize galbonolide B , indicating that galGHIJK is involved in the biosynthesis of galbonolide A. A disruption mutant of orf4 is severely impaired in the production of both galbonolides A and B. These results indicate that galGHIJK and the KAS genes are involved in the biosynthesis of galbonolides , although they are not colocalized with a multimodular PKS gene cluster .
	manualset3
120606	12	404873	5	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A galI-disruption mutant ( SK-galI-5 ) is unable to produce galbonolide A , but can synthesize galbonolide B , indicating that galGHIJK is involved in the biosynthesis of galbonolide A. A disruption mutant of orf4 is severely impaired in the production of both galbonolides A and B. These results indicate that galGHIJK and the KAS genes are involved in the biosynthesis of galbonolides , although they are not colocalized with a multimodular PKS gene cluster .
	manualset3
120607	13	404873	5	NULL	NULL	0	NULL	 galGHIJK gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A galI-disruption mutant ( SK-galI-5 ) is unable to produce galbonolide A , but can synthesize galbonolide B , indicating that galGHIJK is involved in the biosynthesis of galbonolide A. A disruption mutant of orf4 is severely impaired in the production of both galbonolides A and B. These results indicate that galGHIJK and the KAS genes are involved in the biosynthesis of galbonolides , although they are not colocalized with a multimodular PKS gene cluster .
	manualset3
120608	14	404873	5	NULL	NULL	0	NULL	KAS gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A galI-disruption mutant ( SK-galI-5 ) is unable to produce galbonolide A , but can synthesize galbonolide B , indicating that galGHIJK is involved in the biosynthesis of galbonolide A. A disruption mutant of orf4 is severely impaired in the production of both galbonolides A and B. These results indicate that galGHIJK and the KAS genes are involved in the biosynthesis of galbonolides , although they are not colocalized with a multimodular PKS gene cluster .
	manualset3
120609	15	404873	5	NULL	NULL	0	NULL	biosynthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A galI-disruption mutant ( SK-galI-5 ) is unable to produce galbonolide A , but can synthesize galbonolide B , indicating that galGHIJK is involved in the biosynthesis of galbonolide A. A disruption mutant of orf4 is severely impaired in the production of both galbonolides A and B. These results indicate that galGHIJK and the KAS genes are involved in the biosynthesis of galbonolides , although they are not colocalized with a multimodular PKS gene cluster .
	manualset3
120610	16	404873	5	NULL	NULL	0	NULL	galbonolides	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A galI-disruption mutant ( SK-galI-5 ) is unable to produce galbonolide A , but can synthesize galbonolide B , indicating that galGHIJK is involved in the biosynthesis of galbonolide A. A disruption mutant of orf4 is severely impaired in the production of both galbonolides A and B. These results indicate that galGHIJK and the KAS genes are involved in the biosynthesis of galbonolides , although they are not colocalized with a multimodular PKS gene cluster .
	manualset3
120611	17	404873	5	NULL	NULL	0	NULL	multimodular PKS gene cluster	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A galI-disruption mutant ( SK-galI-5 ) is unable to produce galbonolide A , but can synthesize galbonolide B , indicating that galGHIJK is involved in the biosynthesis of galbonolide A. A disruption mutant of orf4 is severely impaired in the production of both galbonolides A and B. These results indicate that galGHIJK and the KAS genes are involved in the biosynthesis of galbonolides , although they are not colocalized with a multimodular PKS gene cluster .
	manualset3
120612	1	404874	5	NULL	NULL	0	NULL	advantages	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly , the advantages offered by the various possible placement sites of the catheter -- i.e. , the II duodenal portion and beyond the ligament of Treitx -- are discussed , together with its different uses according to clinical symptoms : its best location is beyond the ligament of Treitz in subocclusions , versus in the II duodenal portion if tumors or other duodenal conditions are suspected .
	manualset3
120613	2	404874	5	NULL	NULL	0	NULL	possible placement sites	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly , the advantages offered by the various possible placement sites of the catheter -- i.e. , the II duodenal portion and beyond the ligament of Treitx -- are discussed , together with its different uses according to clinical symptoms : its best location is beyond the ligament of Treitz in subocclusions , versus in the II duodenal portion if tumors or other duodenal conditions are suspected .
	manualset3
120614	3	404874	5	NULL	NULL	0	NULL	catheter	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly , the advantages offered by the various possible placement sites of the catheter -- i.e. , the II duodenal portion and beyond the ligament of Treitx -- are discussed , together with its different uses according to clinical symptoms : its best location is beyond the ligament of Treitz in subocclusions , versus in the II duodenal portion if tumors or other duodenal conditions are suspected .
	manualset3
120615	4	404874	5	NULL	NULL	0	NULL	II duodenal portion	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly , the advantages offered by the various possible placement sites of the catheter -- i.e. , the II duodenal portion and beyond the ligament of Treitx -- are discussed , together with its different uses according to clinical symptoms : its best location is beyond the ligament of Treitz in subocclusions , versus in the II duodenal portion if tumors or other duodenal conditions are suspected .
	manualset3
120616	5	404874	5	NULL	NULL	0	NULL	ligament of Treitx	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly , the advantages offered by the various possible placement sites of the catheter -- i.e. , the II duodenal portion and beyond the ligament of Treitx -- are discussed , together with its different uses according to clinical symptoms : its best location is beyond the ligament of Treitz in subocclusions , versus in the II duodenal portion if tumors or other duodenal conditions are suspected .
	manualset3
120617	6	404874	5	NULL	NULL	0	NULL	uses	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly , the advantages offered by the various possible placement sites of the catheter -- i.e. , the II duodenal portion and beyond the ligament of Treitx -- are discussed , together with its different uses according to clinical symptoms : its best location is beyond the ligament of Treitz in subocclusions , versus in the II duodenal portion if tumors or other duodenal conditions are suspected .
	manualset3
120618	7	404874	5	NULL	NULL	0	NULL	clinical symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly , the advantages offered by the various possible placement sites of the catheter -- i.e. , the II duodenal portion and beyond the ligament of Treitx -- are discussed , together with its different uses according to clinical symptoms : its best location is beyond the ligament of Treitz in subocclusions , versus in the II duodenal portion if tumors or other duodenal conditions are suspected .
	manualset3
120619	8	404874	5	NULL	NULL	0	NULL	best location	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly , the advantages offered by the various possible placement sites of the catheter -- i.e. , the II duodenal portion and beyond the ligament of Treitx -- are discussed , together with its different uses according to clinical symptoms : its best location is beyond the ligament of Treitz in subocclusions , versus in the II duodenal portion if tumors or other duodenal conditions are suspected .
	manualset3
120620	9	404874	5	NULL	NULL	0	NULL	ligament of Treitz	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly , the advantages offered by the various possible placement sites of the catheter -- i.e. , the II duodenal portion and beyond the ligament of Treitx -- are discussed , together with its different uses according to clinical symptoms : its best location is beyond the ligament of Treitz in subocclusions , versus in the II duodenal portion if tumors or other duodenal conditions are suspected .
	manualset3
120621	10	404874	5	NULL	NULL	0	NULL	subocclusions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly , the advantages offered by the various possible placement sites of the catheter -- i.e. , the II duodenal portion and beyond the ligament of Treitx -- are discussed , together with its different uses according to clinical symptoms : its best location is beyond the ligament of Treitz in subocclusions , versus in the II duodenal portion if tumors or other duodenal conditions are suspected .
	manualset3
120622	11	404874	5	NULL	NULL	0	NULL	II duodenal portion	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly , the advantages offered by the various possible placement sites of the catheter -- i.e. , the II duodenal portion and beyond the ligament of Treitx -- are discussed , together with its different uses according to clinical symptoms : its best location is beyond the ligament of Treitz in subocclusions , versus in the II duodenal portion if tumors or other duodenal conditions are suspected .
	manualset3
120623	12	404874	5	NULL	NULL	0	NULL	tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly , the advantages offered by the various possible placement sites of the catheter -- i.e. , the II duodenal portion and beyond the ligament of Treitx -- are discussed , together with its different uses according to clinical symptoms : its best location is beyond the ligament of Treitz in subocclusions , versus in the II duodenal portion if tumors or other duodenal conditions are suspected .
	manualset3
120624	13	404874	5	NULL	NULL	0	NULL	duodenal conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly , the advantages offered by the various possible placement sites of the catheter -- i.e. , the II duodenal portion and beyond the ligament of Treitx -- are discussed , together with its different uses according to clinical symptoms : its best location is beyond the ligament of Treitz in subocclusions , versus in the II duodenal portion if tumors or other duodenal conditions are suspected .
	manualset3
120625	1	404875	5	NULL	NULL	0	NULL	medical student programs	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly challenging will be restructuring and funding medical student programs in primary care , given a nearly certain requirement that more than 50 % of medical school graduates enter primary care disciplines .
	manualset3
120626	2	404875	5	NULL	NULL	0	NULL	primary care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly challenging will be restructuring and funding medical student programs in primary care , given a nearly certain requirement that more than 50 % of medical school graduates enter primary care disciplines .
	manualset3
120627	3	404875	5	NULL	NULL	0	NULL	requirement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly challenging will be restructuring and funding medical student programs in primary care , given a nearly certain requirement that more than 50 % of medical school graduates enter primary care disciplines .
	manualset3
120628	4	404875	5	NULL	NULL	0	NULL	50 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly challenging will be restructuring and funding medical student programs in primary care , given a nearly certain requirement that more than 50 % of medical school graduates enter primary care disciplines .
	manualset3
120629	5	404875	5	NULL	NULL	0	NULL	medical school graduates	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly challenging will be restructuring and funding medical student programs in primary care , given a nearly certain requirement that more than 50 % of medical school graduates enter primary care disciplines .
	manualset3
120630	6	404875	5	NULL	NULL	0	NULL	primary care disciplines	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly challenging will be restructuring and funding medical student programs in primary care , given a nearly certain requirement that more than 50 % of medical school graduates enter primary care disciplines .
	manualset3
120631	1	404876	5	NULL	NULL	0	NULL	physician	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly should the physician be concerned with prenatal care , metabolic disorders , increasing numbers of the `` battered child syndrome , '' genetic counseling , psychotherapy and counseling for parent as well as child .
	manualset3
120632	2	404876	5	NULL	NULL	0	NULL	prenatal care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly should the physician be concerned with prenatal care , metabolic disorders , increasing numbers of the `` battered child syndrome , '' genetic counseling , psychotherapy and counseling for parent as well as child .
	manualset3
120633	3	404876	5	NULL	NULL	0	NULL	metabolic disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly should the physician be concerned with prenatal care , metabolic disorders , increasing numbers of the `` battered child syndrome , '' genetic counseling , psychotherapy and counseling for parent as well as child .
	manualset3
120634	4	404876	5	NULL	NULL	0	NULL	battered child syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly should the physician be concerned with prenatal care , metabolic disorders , increasing numbers of the `` battered child syndrome , '' genetic counseling , psychotherapy and counseling for parent as well as child .
	manualset3
120635	5	404876	5	NULL	NULL	0	NULL	genetic counseling	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly should the physician be concerned with prenatal care , metabolic disorders , increasing numbers of the `` battered child syndrome , '' genetic counseling , psychotherapy and counseling for parent as well as child .
	manualset3
120636	6	404876	5	NULL	NULL	0	NULL	psychotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly should the physician be concerned with prenatal care , metabolic disorders , increasing numbers of the `` battered child syndrome , '' genetic counseling , psychotherapy and counseling for parent as well as child .
	manualset3
120637	7	404876	5	NULL	NULL	0	NULL	counseling	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly should the physician be concerned with prenatal care , metabolic disorders , increasing numbers of the `` battered child syndrome , '' genetic counseling , psychotherapy and counseling for parent as well as child .
	manualset3
120638	8	404876	5	NULL	NULL	0	NULL	parent	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly should the physician be concerned with prenatal care , metabolic disorders , increasing numbers of the `` battered child syndrome , '' genetic counseling , psychotherapy and counseling for parent as well as child .
	manualset3
120639	9	404876	5	NULL	NULL	0	NULL	child	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly should the physician be concerned with prenatal care , metabolic disorders , increasing numbers of the `` battered child syndrome , '' genetic counseling , psychotherapy and counseling for parent as well as child .
	manualset3
120640	1	404877	5	NULL	NULL	0	NULL	sleep disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly so with those diagnosed with sleep disorders with significant motility or long catatonic periods of wakefulness during sleep .
	manualset3
120641	2	404877	5	NULL	NULL	0	NULL	significant motility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly so with those diagnosed with sleep disorders with significant motility or long catatonic periods of wakefulness during sleep .
	manualset3
120642	3	404877	5	NULL	NULL	0	NULL	long catatonic periods of wakefulness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly so with those diagnosed with sleep disorders with significant motility or long catatonic periods of wakefulness during sleep .
	manualset3
120643	4	404877	5	NULL	NULL	0	NULL	sleep	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Particularly so with those diagnosed with sleep disorders with significant motility or long catatonic periods of wakefulness during sleep .
	manualset3
120644	1	404878	5	NULL	NULL	0	NULL	Parturition control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Parturition control in sows with a prostaglandin analog ( alfaprostol ) .
	manualset3
120645	2	404878	5	NULL	NULL	0	NULL	sows	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Parturition control in sows with a prostaglandin analog ( alfaprostol ) .
	manualset3
120646	3	404878	5	NULL	NULL	0	NULL	prostaglandin analog ( alfaprostol )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Parturition control in sows with a prostaglandin analog ( alfaprostol ) .
	manualset3
120647	1	404879	5	NULL	NULL	0	NULL	Parvalbumin-immunoreactive neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Parvalbumin-immunoreactive neurons in the rat neostriatum : a light and electron microscopic study .
	manualset3
120648	2	404879	5	NULL	NULL	0	NULL	rat neostriatum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Parvalbumin-immunoreactive neurons in the rat neostriatum : a light and electron microscopic study .
	manualset3
120649	3	404879	5	NULL	NULL	0	NULL	light and electron microscopic study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parvalbumin-immunoreactive neurons in the rat neostriatum : a light and electron microscopic study .
	manualset3
122302	1	404880	5	NULL	NULL	0	NULL	laser 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Passively mode-locked Yb & lt ; sup & gt ; 3 + & lt ; / sup & gt ; : Sc & lt ; sub & gt ; 2 & lt ; / sub & gt ; SiO & lt ; sub & gt ; 5 & lt ; / sub & gt ; laser with reflection-type single-walled carbon nanotube absorber .
	manualset3
122303	2	404880	5	NULL	NULL	0	NULL	reflection-type single-walled carbon nanotube absorber	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Passively mode-locked Yb & lt ; sup & gt ; 3 + & lt ; / sup & gt ; : Sc & lt ; sub & gt ; 2 & lt ; / sub & gt ; SiO & lt ; sub & gt ; 5 & lt ; / sub & gt ; laser with reflection-type single-walled carbon nanotube absorber .
	manualset3
120650	1	404881	5	NULL	NULL	0	NULL	chloroplast transformation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Past studies in chloroplast transformation used qualitative Southern blots to evaluate indirectly transgene copy number , whereas we used real-time PCR for the first time to establish homoplasmy and estimate transgene copy number and transcript levels .
	manualset3
120651	2	404881	5	NULL	NULL	0	NULL	qualitative Southern blots 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Past studies in chloroplast transformation used qualitative Southern blots to evaluate indirectly transgene copy number , whereas we used real-time PCR for the first time to establish homoplasmy and estimate transgene copy number and transcript levels .
	manualset3
120652	3	404881	5	NULL	NULL	0	NULL	transgene copy number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Past studies in chloroplast transformation used qualitative Southern blots to evaluate indirectly transgene copy number , whereas we used real-time PCR for the first time to establish homoplasmy and estimate transgene copy number and transcript levels .
	manualset3
120653	4	404881	5	NULL	NULL	0	NULL	real-time PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Past studies in chloroplast transformation used qualitative Southern blots to evaluate indirectly transgene copy number , whereas we used real-time PCR for the first time to establish homoplasmy and estimate transgene copy number and transcript levels .
	manualset3
120654	5	404881	5	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Past studies in chloroplast transformation used qualitative Southern blots to evaluate indirectly transgene copy number , whereas we used real-time PCR for the first time to establish homoplasmy and estimate transgene copy number and transcript levels .
	manualset3
120655	6	404881	5	NULL	NULL	0	NULL	homoplasmy 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Past studies in chloroplast transformation used qualitative Southern blots to evaluate indirectly transgene copy number , whereas we used real-time PCR for the first time to establish homoplasmy and estimate transgene copy number and transcript levels .
	manualset3
120656	7	404881	5	NULL	NULL	0	NULL	transgene copy number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Past studies in chloroplast transformation used qualitative Southern blots to evaluate indirectly transgene copy number , whereas we used real-time PCR for the first time to establish homoplasmy and estimate transgene copy number and transcript levels .
	manualset3
120657	8	404881	5	NULL	NULL	0	NULL	transcript levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Past studies in chloroplast transformation used qualitative Southern blots to evaluate indirectly transgene copy number , whereas we used real-time PCR for the first time to establish homoplasmy and estimate transgene copy number and transcript levels .
	manualset3
120658	1	404882	5	NULL	NULL	0	NULL	Pasteurella multocida infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pasteurella multocida infection following cisplatin and 5-fluorouracil chemotherapy .
	manualset3
120659	3	404882	5	NULL	NULL	NULL	NULL	 5-fluorouracil chemotherapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pasteurella multocida infection following cisplatin and 5-fluorouracil chemotherapy .
	manualset3
123766	2	404882	5	NULL	NULL	0	NULL	cisplatin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pasteurella multocida infection following cisplatin and 5-fluorouracil chemotherapy .
	manualset3
120660	1	404883	5	NULL	NULL	0	NULL	Patch-clamp recording	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patch-clamp recording of light responses can be combined with dye filling to reveal the morphology and to check for gap junction-mediated dye coupling to neighboring cells , so that the target cell can by studied on different experimental levels .
	manualset3
120661	2	404883	5	NULL	NULL	0	NULL	light responses	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patch-clamp recording of light responses can be combined with dye filling to reveal the morphology and to check for gap junction-mediated dye coupling to neighboring cells , so that the target cell can by studied on different experimental levels .
	manualset3
120662	3	404883	5	NULL	NULL	0	NULL	dye filling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patch-clamp recording of light responses can be combined with dye filling to reveal the morphology and to check for gap junction-mediated dye coupling to neighboring cells , so that the target cell can by studied on different experimental levels .
	manualset3
120663	4	404883	5	NULL	NULL	0	NULL	morphology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patch-clamp recording of light responses can be combined with dye filling to reveal the morphology and to check for gap junction-mediated dye coupling to neighboring cells , so that the target cell can by studied on different experimental levels .
	manualset3
120664	5	404883	5	NULL	NULL	0	NULL	gap junction-mediated dye coupling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patch-clamp recording of light responses can be combined with dye filling to reveal the morphology and to check for gap junction-mediated dye coupling to neighboring cells , so that the target cell can by studied on different experimental levels .
	manualset3
120665	6	404883	5	NULL	NULL	0	NULL	neighboring cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Patch-clamp recording of light responses can be combined with dye filling to reveal the morphology and to check for gap junction-mediated dye coupling to neighboring cells , so that the target cell can by studied on different experimental levels .
	manualset3
120666	7	404883	5	NULL	NULL	0	NULL	target cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Patch-clamp recording of light responses can be combined with dye filling to reveal the morphology and to check for gap junction-mediated dye coupling to neighboring cells , so that the target cell can by studied on different experimental levels .
	manualset3
120667	8	404883	5	NULL	NULL	0	NULL	experimental levels	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patch-clamp recording of light responses can be combined with dye filling to reveal the morphology and to check for gap junction-mediated dye coupling to neighboring cells , so that the target cell can by studied on different experimental levels .
	manualset3
120668	1	404884	5	NULL	NULL	0	NULL	Patch testing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patch testing with protective gloves should always be used when patients develop prolonged hand dermatitis and where the possibility of glove eczema exists .
	manualset3
120669	2	404884	5	NULL	NULL	0	NULL	protective gloves	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Patch testing with protective gloves should always be used when patients develop prolonged hand dermatitis and where the possibility of glove eczema exists .
	manualset3
120670	3	404884	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patch testing with protective gloves should always be used when patients develop prolonged hand dermatitis and where the possibility of glove eczema exists .
	manualset3
120671	4	404884	5	NULL	NULL	0	NULL	hand dermatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patch testing with protective gloves should always be used when patients develop prolonged hand dermatitis and where the possibility of glove eczema exists .
	manualset3
120672	5	404884	5	NULL	NULL	0	NULL	possibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patch testing with protective gloves should always be used when patients develop prolonged hand dermatitis and where the possibility of glove eczema exists .
	manualset3
120673	6	404884	5	NULL	NULL	0	NULL	glove eczema 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patch testing with protective gloves should always be used when patients develop prolonged hand dermatitis and where the possibility of glove eczema exists .
	manualset3
120674	1	404885	5	NULL	NULL	0	NULL	Patency 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patency and normal renin levels were achieved within two months in 2 patients .
	manualset3
120675	2	404885	5	NULL	NULL	0	NULL	normal renin levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patency and normal renin levels were achieved within two months in 2 patients .
	manualset3
120676	3	404885	5	NULL	NULL	0	NULL	two months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Patency and normal renin levels were achieved within two months in 2 patients .
	manualset3
120677	4	404885	5	NULL	NULL	0	NULL	 2 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patency and normal renin levels were achieved within two months in 2 patients .
	manualset3
120678	1	404886	5	NULL	NULL	0	NULL	Patency 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patency of the valved conduits was confirmed during the initial procedure , and there was no incidence of paraplegia postoperatively .
	manualset3
120679	2	404886	5	NULL	NULL	0	NULL	valved conduits 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Patency of the valved conduits was confirmed during the initial procedure , and there was no incidence of paraplegia postoperatively .
	manualset3
120680	3	404886	5	NULL	NULL	0	NULL	initial procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patency of the valved conduits was confirmed during the initial procedure , and there was no incidence of paraplegia postoperatively .
	manualset3
120681	4	404886	5	NULL	NULL	0	NULL	incidence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patency of the valved conduits was confirmed during the initial procedure , and there was no incidence of paraplegia postoperatively .
	manualset3
120682	5	404886	5	NULL	NULL	0	NULL	paraplegia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patency of the valved conduits was confirmed during the initial procedure , and there was no incidence of paraplegia postoperatively .
	manualset3
120683	1	404887	5	NULL	NULL	NULL	NULL	Patent blue ( PB ) dye 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patent blue ( PB ) dye has been successfully used worldwide in breast and cervix surgeries with few complications .
	manualset3
120684	2	404887	5	NULL	NULL	0	NULL	worldwide 	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Patent blue ( PB ) dye has been successfully used worldwide in breast and cervix surgeries with few complications .
	manualset3
120685	3	404887	5	NULL	NULL	0	NULL	breast surgeries 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patent blue ( PB ) dye has been successfully used worldwide in breast and cervix surgeries with few complications .
	manualset3
120686	4	404887	5	NULL	NULL	0	NULL	cervix surgeries 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patent blue ( PB ) dye has been successfully used worldwide in breast and cervix surgeries with few complications .
	manualset3
120687	5	404887	5	NULL	NULL	0	NULL	complications 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patent blue ( PB ) dye has been successfully used worldwide in breast and cervix surgeries with few complications .
	manualset3
120688	1	404888	5	NULL	NULL	0	NULL	Patent ductus arteriosus ( PDA ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patent ductus arteriosus ( PDA ) is a common congenital heart disease that results when the ductus arteriosus , a muscular artery , fails to remodel and close after birth .
	manualset3
120689	2	404888	5	NULL	NULL	0	NULL	congenital heart disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patent ductus arteriosus ( PDA ) is a common congenital heart disease that results when the ductus arteriosus , a muscular artery , fails to remodel and close after birth .
	manualset3
120690	3	404888	5	NULL	NULL	0	NULL	results 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patent ductus arteriosus ( PDA ) is a common congenital heart disease that results when the ductus arteriosus , a muscular artery , fails to remodel and close after birth .
	manualset3
120691	4	404888	5	NULL	NULL	0	NULL	ductus arteriosus , a muscular artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Patent ductus arteriosus ( PDA ) is a common congenital heart disease that results when the ductus arteriosus , a muscular artery , fails to remodel and close after birth .
	manualset3
120692	5	404888	5	NULL	NULL	0	NULL	remodel 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Patent ductus arteriosus ( PDA ) is a common congenital heart disease that results when the ductus arteriosus , a muscular artery , fails to remodel and close after birth .
	manualset3
120693	6	404888	5	NULL	NULL	0	NULL	birth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Patent ductus arteriosus ( PDA ) is a common congenital heart disease that results when the ductus arteriosus , a muscular artery , fails to remodel and close after birth .
	manualset3
120694	1	404889	5	NULL	NULL	0	NULL	Patent ductus arteriosus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patent ductus arteriosus and its treatment as risk factors for neonatal and neurodevelopmental morbidity .
	manualset3
120695	2	404889	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patent ductus arteriosus and its treatment as risk factors for neonatal and neurodevelopmental morbidity .
	manualset3
120696	3	404889	5	NULL	NULL	0	NULL	risk factors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patent ductus arteriosus and its treatment as risk factors for neonatal and neurodevelopmental morbidity .
	manualset3
120697	4	404889	5	NULL	NULL	0	NULL	neonatal morbidity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patent ductus arteriosus and its treatment as risk factors for neonatal and neurodevelopmental morbidity .
	manualset3
120698	5	404889	5	NULL	NULL	0	NULL	neurodevelopmental morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patent ductus arteriosus and its treatment as risk factors for neonatal and neurodevelopmental morbidity .
	manualset3
120699	1	404890	5	NULL	NULL	0	NULL	Paternally behaving males 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Paternally behaving males subjected to chronic exposure to pups were incapable of secreting nocturnal surges of prolactin characteristic of the pseudopregnant female .
	manualset3
120700	2	404890	5	NULL	NULL	0	NULL	chronic exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Paternally behaving males subjected to chronic exposure to pups were incapable of secreting nocturnal surges of prolactin characteristic of the pseudopregnant female .
	manualset3
120701	3	404890	5	NULL	NULL	0	NULL	pups 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Paternally behaving males subjected to chronic exposure to pups were incapable of secreting nocturnal surges of prolactin characteristic of the pseudopregnant female .
	manualset3
120702	4	404890	5	NULL	NULL	0	NULL	nocturnal surges 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Paternally behaving males subjected to chronic exposure to pups were incapable of secreting nocturnal surges of prolactin characteristic of the pseudopregnant female .
	manualset3
120703	5	404890	5	NULL	NULL	0	NULL	prolactin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Paternally behaving males subjected to chronic exposure to pups were incapable of secreting nocturnal surges of prolactin characteristic of the pseudopregnant female .
	manualset3
120704	6	404890	5	NULL	NULL	0	NULL	pseudopregnant female	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Paternally behaving males subjected to chronic exposure to pups were incapable of secreting nocturnal surges of prolactin characteristic of the pseudopregnant female .
	manualset3
120705	1	404891	5	NULL	NULL	0	NULL	Path-integral Monte Carlo simulation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Path-integral Monte Carlo simulation of nu3 vibrational shifts for CO2 in ( He ) n clusters critically tests the He-CO2 potential energy surface .
	manualset3
120706	2	404891	5	NULL	NULL	0	NULL	nu3 vibrational shifts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Path-integral Monte Carlo simulation of nu3 vibrational shifts for CO2 in ( He ) n clusters critically tests the He-CO2 potential energy surface .
	manualset3
120707	3	404891	5	NULL	NULL	0	NULL	CO2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Path-integral Monte Carlo simulation of nu3 vibrational shifts for CO2 in ( He ) n clusters critically tests the He-CO2 potential energy surface .
	manualset3
120708	4	404891	5	NULL	NULL	0	NULL	( He ) n clusters	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Path-integral Monte Carlo simulation of nu3 vibrational shifts for CO2 in ( He ) n clusters critically tests the He-CO2 potential energy surface .
	manualset3
120709	5	404891	5	NULL	NULL	0	NULL	tests 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Path-integral Monte Carlo simulation of nu3 vibrational shifts for CO2 in ( He ) n clusters critically tests the He-CO2 potential energy surface .
	manualset3
120710	6	404891	5	NULL	NULL	0	NULL	He-CO2 potential energy surface	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Path-integral Monte Carlo simulation of nu3 vibrational shifts for CO2 in ( He ) n clusters critically tests the He-CO2 potential energy surface .
	manualset3
120712	1	404892	5	NULL	NULL	0	NULL	gene probe	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A gene probe constructed from the `` alkB '' PCR fragment from strain Q15 did hybridize with the alkB PCR fragments from most of the psychrotrophic alkane biodegraders , indicating that the alkB primers may be amplifying another gene ( s ) , perhaps with low homology to P. oleovorans alkB , which may be involved in the biodegradation of both short chain ( dodecane ) and longer chain alkanes ( hexadecane , octacosane ) .
	manualset3
120713	2	404892	5	NULL	NULL	0	NULL	 `` alkB '' PCR fragment	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A gene probe constructed from the `` alkB '' PCR fragment from strain Q15 did hybridize with the alkB PCR fragments from most of the psychrotrophic alkane biodegraders , indicating that the alkB primers may be amplifying another gene ( s ) , perhaps with low homology to P. oleovorans alkB , which may be involved in the biodegradation of both short chain ( dodecane ) and longer chain alkanes ( hexadecane , octacosane ) .
	manualset3
120714	3	404892	5	NULL	NULL	0	NULL	strain Q15	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A gene probe constructed from the `` alkB '' PCR fragment from strain Q15 did hybridize with the alkB PCR fragments from most of the psychrotrophic alkane biodegraders , indicating that the alkB primers may be amplifying another gene ( s ) , perhaps with low homology to P. oleovorans alkB , which may be involved in the biodegradation of both short chain ( dodecane ) and longer chain alkanes ( hexadecane , octacosane ) .
	manualset3
120715	4	404892	5	NULL	NULL	0	NULL	alkB PCR fragments	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A gene probe constructed from the `` alkB '' PCR fragment from strain Q15 did hybridize with the alkB PCR fragments from most of the psychrotrophic alkane biodegraders , indicating that the alkB primers may be amplifying another gene ( s ) , perhaps with low homology to P. oleovorans alkB , which may be involved in the biodegradation of both short chain ( dodecane ) and longer chain alkanes ( hexadecane , octacosane ) .
	manualset3
120716	5	404892	5	NULL	NULL	0	NULL	psychrotrophic alkane biodegraders	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A gene probe constructed from the `` alkB '' PCR fragment from strain Q15 did hybridize with the alkB PCR fragments from most of the psychrotrophic alkane biodegraders , indicating that the alkB primers may be amplifying another gene ( s ) , perhaps with low homology to P. oleovorans alkB , which may be involved in the biodegradation of both short chain ( dodecane ) and longer chain alkanes ( hexadecane , octacosane ) .
	manualset3
120717	6	404892	5	NULL	NULL	0	NULL	alkB primers 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A gene probe constructed from the `` alkB '' PCR fragment from strain Q15 did hybridize with the alkB PCR fragments from most of the psychrotrophic alkane biodegraders , indicating that the alkB primers may be amplifying another gene ( s ) , perhaps with low homology to P. oleovorans alkB , which may be involved in the biodegradation of both short chain ( dodecane ) and longer chain alkanes ( hexadecane , octacosane ) .
	manualset3
120718	7	404892	5	NULL	NULL	0	NULL	gene ( s )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A gene probe constructed from the `` alkB '' PCR fragment from strain Q15 did hybridize with the alkB PCR fragments from most of the psychrotrophic alkane biodegraders , indicating that the alkB primers may be amplifying another gene ( s ) , perhaps with low homology to P. oleovorans alkB , which may be involved in the biodegradation of both short chain ( dodecane ) and longer chain alkanes ( hexadecane , octacosane ) .
	manualset3
120719	8	404892	5	NULL	NULL	NULL	NULL	low homology	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A gene probe constructed from the `` alkB '' PCR fragment from strain Q15 did hybridize with the alkB PCR fragments from most of the psychrotrophic alkane biodegraders , indicating that the alkB primers may be amplifying another gene ( s ) , perhaps with low homology to P. oleovorans alkB , which may be involved in the biodegradation of both short chain ( dodecane ) and longer chain alkanes ( hexadecane , octacosane ) .
	manualset3
120720	9	404892	5	NULL	NULL	0	NULL	P. oleovorans alkB	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A gene probe constructed from the `` alkB '' PCR fragment from strain Q15 did hybridize with the alkB PCR fragments from most of the psychrotrophic alkane biodegraders , indicating that the alkB primers may be amplifying another gene ( s ) , perhaps with low homology to P. oleovorans alkB , which may be involved in the biodegradation of both short chain ( dodecane ) and longer chain alkanes ( hexadecane , octacosane ) .
	manualset3
120721	10	404892	5	NULL	NULL	0	NULL	biodegradation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A gene probe constructed from the `` alkB '' PCR fragment from strain Q15 did hybridize with the alkB PCR fragments from most of the psychrotrophic alkane biodegraders , indicating that the alkB primers may be amplifying another gene ( s ) , perhaps with low homology to P. oleovorans alkB , which may be involved in the biodegradation of both short chain ( dodecane ) and longer chain alkanes ( hexadecane , octacosane ) .
	manualset3
120722	11	404892	5	NULL	NULL	0	NULL	short chain ( dodecane ) alkanes 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A gene probe constructed from the `` alkB '' PCR fragment from strain Q15 did hybridize with the alkB PCR fragments from most of the psychrotrophic alkane biodegraders , indicating that the alkB primers may be amplifying another gene ( s ) , perhaps with low homology to P. oleovorans alkB , which may be involved in the biodegradation of both short chain ( dodecane ) and longer chain alkanes ( hexadecane , octacosane ) .
	manualset3
120723	12	404892	5	NULL	NULL	0	NULL	 longer chain alkanes ( hexadecane , octacosane ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A gene probe constructed from the `` alkB '' PCR fragment from strain Q15 did hybridize with the alkB PCR fragments from most of the psychrotrophic alkane biodegraders , indicating that the alkB primers may be amplifying another gene ( s ) , perhaps with low homology to P. oleovorans alkB , which may be involved in the biodegradation of both short chain ( dodecane ) and longer chain alkanes ( hexadecane , octacosane ) .
	manualset3
120724	1	404893	5	NULL	NULL	0	NULL	Pathoadaptive mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathoadaptive mutations improve the fitness of pathogenic species by modification of traits that interfere with factors ( virulence and ancestral ) required for survival in host tissues .
	manualset3
120725	2	404893	5	NULL	NULL	0	NULL	fitness 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathoadaptive mutations improve the fitness of pathogenic species by modification of traits that interfere with factors ( virulence and ancestral ) required for survival in host tissues .
	manualset3
120726	3	404893	5	NULL	NULL	0	NULL	pathogenic species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathoadaptive mutations improve the fitness of pathogenic species by modification of traits that interfere with factors ( virulence and ancestral ) required for survival in host tissues .
	manualset3
120727	4	404893	5	NULL	NULL	0	NULL	modification 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathoadaptive mutations improve the fitness of pathogenic species by modification of traits that interfere with factors ( virulence and ancestral ) required for survival in host tissues .
	manualset3
120728	5	404893	5	NULL	NULL	0	NULL	traits 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathoadaptive mutations improve the fitness of pathogenic species by modification of traits that interfere with factors ( virulence and ancestral ) required for survival in host tissues .
	manualset3
120729	6	404893	5	NULL	NULL	0	NULL	factors ( virulence and ancestral )	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathoadaptive mutations improve the fitness of pathogenic species by modification of traits that interfere with factors ( virulence and ancestral ) required for survival in host tissues .
	manualset3
120730	7	404893	5	NULL	NULL	0	NULL	survival 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathoadaptive mutations improve the fitness of pathogenic species by modification of traits that interfere with factors ( virulence and ancestral ) required for survival in host tissues .
	manualset3
120731	8	404893	5	NULL	NULL	0	NULL	host tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathoadaptive mutations improve the fitness of pathogenic species by modification of traits that interfere with factors ( virulence and ancestral ) required for survival in host tissues .
	manualset3
120732	1	404894	5	NULL	NULL	0	NULL	Pathogen-associated molecular pattern-induced mitochondrial membrane depolarization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathogen-associated molecular pattern-induced mitochondrial membrane depolarization in the earthworm Eisenia hortensis .
	manualset3
120733	2	404894	5	NULL	NULL	0	NULL	earthworm Eisenia hortensis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathogen-associated molecular pattern-induced mitochondrial membrane depolarization in the earthworm Eisenia hortensis .
	manualset3
120734	1	404895	5	NULL	NULL	0	NULL	Pathogen elimination 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathogen elimination was dependent on the interferon gamma inducible-p47 GTPase , IGTP , required PI3K activity , and was preceded by PV membrane indentation , vesiculation , disruption , and , surprisingly , stripping of the parasite plasma membrane .
	manualset3
120735	2	404895	5	NULL	NULL	NULL	NULL	interferon gamma inducible-p47 GTPase , IGTP	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pathogen elimination was dependent on the interferon gamma inducible-p47 GTPase , IGTP , required PI3K activity , and was preceded by PV membrane indentation , vesiculation , disruption , and , surprisingly , stripping of the parasite plasma membrane .
	manualset3
120737	3	404895	5	NULL	NULL	NULL	NULL	 PI3K activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pathogen elimination was dependent on the interferon gamma inducible-p47 GTPase , IGTP , required PI3K activity , and was preceded by PV membrane indentation , vesiculation , disruption , and , surprisingly , stripping of the parasite plasma membrane .
	manualset3
120738	4	404895	5	NULL	NULL	0	NULL	PV membrane indentation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathogen elimination was dependent on the interferon gamma inducible-p47 GTPase , IGTP , required PI3K activity , and was preceded by PV membrane indentation , vesiculation , disruption , and , surprisingly , stripping of the parasite plasma membrane .
	manualset3
120739	5	404895	5	NULL	NULL	0	NULL	vesiculation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathogen elimination was dependent on the interferon gamma inducible-p47 GTPase , IGTP , required PI3K activity , and was preceded by PV membrane indentation , vesiculation , disruption , and , surprisingly , stripping of the parasite plasma membrane .
	manualset3
120740	6	404895	5	NULL	NULL	0	NULL	disruption 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathogen elimination was dependent on the interferon gamma inducible-p47 GTPase , IGTP , required PI3K activity , and was preceded by PV membrane indentation , vesiculation , disruption , and , surprisingly , stripping of the parasite plasma membrane .
	manualset3
120741	7	404895	5	NULL	NULL	NULL	NULL	stripping of the parasite plasma membrane	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pathogen elimination was dependent on the interferon gamma inducible-p47 GTPase , IGTP , required PI3K activity , and was preceded by PV membrane indentation , vesiculation , disruption , and , surprisingly , stripping of the parasite plasma membrane .
	manualset3
120742	1	404896	5	NULL	NULL	0	NULL	Pathogenesis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathogenesis and pathology of cobalt cardiomyopathy .
	manualset3
120743	2	404896	5	NULL	NULL	0	NULL	pathology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathogenesis and pathology of cobalt cardiomyopathy .
	manualset3
120744	3	404896	5	NULL	NULL	0	NULL	cobalt cardiomyopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathogenesis and pathology of cobalt cardiomyopathy .
	manualset3
120745	1	404897	5	NULL	NULL	0	NULL	Pathogenesis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathogenesis mediated by Shigella flexneri requires invasion of the gastrointestinal epithelium .
	manualset3
120746	2	404897	5	NULL	NULL	0	NULL	Shigella flexneri	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathogenesis mediated by Shigella flexneri requires invasion of the gastrointestinal epithelium .
	manualset3
120747	3	404897	5	NULL	NULL	0	NULL	invasion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathogenesis mediated by Shigella flexneri requires invasion of the gastrointestinal epithelium .
	manualset3
120748	4	404897	5	NULL	NULL	NULL	NULL	gastrointestinal epithelium	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pathogenesis mediated by Shigella flexneri requires invasion of the gastrointestinal epithelium .
	manualset3
120749	1	404898	5	NULL	NULL	0	NULL	Pathogenesis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathogenesis of diabetic retinopathy and strategy to develop new therapeutic modalities .
	manualset3
120750	2	404898	5	NULL	NULL	0	NULL	diabetic retinopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathogenesis of diabetic retinopathy and strategy to develop new therapeutic modalities .
	manualset3
120751	3	404898	5	NULL	NULL	0	NULL	strategy 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathogenesis of diabetic retinopathy and strategy to develop new therapeutic modalities .
	manualset3
120752	4	404898	5	NULL	NULL	0	NULL	develop 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathogenesis of diabetic retinopathy and strategy to develop new therapeutic modalities .
	manualset3
120753	5	404898	5	NULL	NULL	NULL	NULL	new therapeutic modalities	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pathogenesis of diabetic retinopathy and strategy to develop new therapeutic modalities .
	manualset3
120754	1	404899	5	NULL	NULL	0	NULL	Pathogenesis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathogenesis of polycystic ovary syndrome : what is the role of obesity ?
	manualset3
120755	2	404899	5	NULL	NULL	0	NULL	polycystic ovary syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathogenesis of polycystic ovary syndrome : what is the role of obesity ?
	manualset3
120756	3	404899	5	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathogenesis of polycystic ovary syndrome : what is the role of obesity ?
	manualset3
120757	4	404899	5	NULL	NULL	0	NULL	obesity 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathogenesis of polycystic ovary syndrome : what is the role of obesity ?
	manualset3
120758	1	404900	5	NULL	NULL	0	NULL	Pathologic examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathologic examination revealed right ovarian clear-cell carcinoma with peritoneal , omental , and fallopian tube metastasis , and conventional clear-cell renal carcinoma .
	manualset3
120759	2	404900	5	NULL	NULL	0	NULL	right ovarian clear-cell carcinoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathologic examination revealed right ovarian clear-cell carcinoma with peritoneal , omental , and fallopian tube metastasis , and conventional clear-cell renal carcinoma .
	manualset3
120760	3	404900	5	NULL	NULL	0	NULL	peritoneal , omental , and fallopian tube metastasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathologic examination revealed right ovarian clear-cell carcinoma with peritoneal , omental , and fallopian tube metastasis , and conventional clear-cell renal carcinoma .
	manualset3
120761	4	404900	5	NULL	NULL	0	NULL	conventional clear-cell renal carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathologic examination revealed right ovarian clear-cell carcinoma with peritoneal , omental , and fallopian tube metastasis , and conventional clear-cell renal carcinoma .
	manualset3
120762	1	404901	5	NULL	NULL	0	NULL	Pathologic staging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathologic staging of the specimens revealed 20 T1 N0 , 10 T2 N0 , 5 T1 N1 , and 6 T2 N1 lesions .
	manualset3
120763	2	404901	5	NULL	NULL	0	NULL	specimens 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathologic staging of the specimens revealed 20 T1 N0 , 10 T2 N0 , 5 T1 N1 , and 6 T2 N1 lesions .
	manualset3
120764	3	404901	5	NULL	NULL	0	NULL	20 T1 N0 lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathologic staging of the specimens revealed 20 T1 N0 , 10 T2 N0 , 5 T1 N1 , and 6 T2 N1 lesions .
	manualset3
120765	4	404901	5	NULL	NULL	NULL	NULL	10 T2 N0 lesions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pathologic staging of the specimens revealed 20 T1 N0 , 10 T2 N0 , 5 T1 N1 , and 6 T2 N1 lesions .
	manualset3
120766	5	404901	5	NULL	NULL	NULL	NULL	5 T1 N1 lesions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pathologic staging of the specimens revealed 20 T1 N0 , 10 T2 N0 , 5 T1 N1 , and 6 T2 N1 lesions .
	manualset3
120767	6	404901	5	NULL	NULL	0	NULL	6 T2 N1 lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathologic staging of the specimens revealed 20 T1 N0 , 10 T2 N0 , 5 T1 N1 , and 6 T2 N1 lesions .
	manualset3
120768	1	404902	5	NULL	NULL	0	NULL	general deficiency 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A general deficiency in omega-3 contributes to the lacking reduction in Schizophrenia , despite early puberty predominates .
	manualset3
120769	2	404902	5	NULL	NULL	0	NULL	omega-3 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A general deficiency in omega-3 contributes to the lacking reduction in Schizophrenia , despite early puberty predominates .
	manualset3
120770	3	404902	5	NULL	NULL	0	NULL	lacking reduction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A general deficiency in omega-3 contributes to the lacking reduction in Schizophrenia , despite early puberty predominates .
	manualset3
120771	4	404902	5	NULL	NULL	0	NULL	Schizophrenia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A general deficiency in omega-3 contributes to the lacking reduction in Schizophrenia , despite early puberty predominates .
	manualset3
120772	5	404902	5	NULL	NULL	0	NULL	early puberty	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A general deficiency in omega-3 contributes to the lacking reduction in Schizophrenia , despite early puberty predominates .
	manualset3
120773	1	404903	5	NULL	NULL	0	NULL	Pathological changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathological changes occurred in the foetus in 2 out of 3 pregnant ewes and the ewe produced a healthy lamb which had antibodies to WSL virus in pre-colostral serum .
	manualset3
120774	2	404903	5	NULL	NULL	0	NULL	foetus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathological changes occurred in the foetus in 2 out of 3 pregnant ewes and the ewe produced a healthy lamb which had antibodies to WSL virus in pre-colostral serum .
	manualset3
120775	3	404903	5	NULL	NULL	0	NULL	2 out of 3	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathological changes occurred in the foetus in 2 out of 3 pregnant ewes and the ewe produced a healthy lamb which had antibodies to WSL virus in pre-colostral serum .
	manualset3
120776	4	404903	5	NULL	NULL	0	NULL	pregnant ewes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathological changes occurred in the foetus in 2 out of 3 pregnant ewes and the ewe produced a healthy lamb which had antibodies to WSL virus in pre-colostral serum .
	manualset3
120777	5	404903	5	NULL	NULL	0	NULL	ewe 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathological changes occurred in the foetus in 2 out of 3 pregnant ewes and the ewe produced a healthy lamb which had antibodies to WSL virus in pre-colostral serum .
	manualset3
120778	6	404903	5	NULL	NULL	0	NULL	healthy lamb	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathological changes occurred in the foetus in 2 out of 3 pregnant ewes and the ewe produced a healthy lamb which had antibodies to WSL virus in pre-colostral serum .
	manualset3
120779	7	404903	5	NULL	NULL	0	NULL	antibodies 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathological changes occurred in the foetus in 2 out of 3 pregnant ewes and the ewe produced a healthy lamb which had antibodies to WSL virus in pre-colostral serum .
	manualset3
120780	8	404903	5	NULL	NULL	0	NULL	WSL virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathological changes occurred in the foetus in 2 out of 3 pregnant ewes and the ewe produced a healthy lamb which had antibodies to WSL virus in pre-colostral serum .
	manualset3
120781	9	404903	5	NULL	NULL	0	NULL	pre-colostral serum 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathological changes occurred in the foetus in 2 out of 3 pregnant ewes and the ewe produced a healthy lamb which had antibodies to WSL virus in pre-colostral serum .
	manualset3
120782	1	404904	5	NULL	NULL	0	NULL	Pathological examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathological examination revealed the characteristic alterations of spongiform encephalopathy , severe in the thalamus , moderate but widely spread in the cerebral cortices , and moderate in the cerebellum .
	manualset3
120783	2	404904	5	NULL	NULL	0	NULL	characteristic alterations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathological examination revealed the characteristic alterations of spongiform encephalopathy , severe in the thalamus , moderate but widely spread in the cerebral cortices , and moderate in the cerebellum .
	manualset3
120784	3	404904	5	NULL	NULL	0	NULL	spongiform encephalopathy 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathological examination revealed the characteristic alterations of spongiform encephalopathy , severe in the thalamus , moderate but widely spread in the cerebral cortices , and moderate in the cerebellum .
	manualset3
120785	4	404904	5	NULL	NULL	0	NULL	thalamus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathological examination revealed the characteristic alterations of spongiform encephalopathy , severe in the thalamus , moderate but widely spread in the cerebral cortices , and moderate in the cerebellum .
	manualset3
120786	5	404904	5	NULL	NULL	0	NULL	cerebral cortices	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathological examination revealed the characteristic alterations of spongiform encephalopathy , severe in the thalamus , moderate but widely spread in the cerebral cortices , and moderate in the cerebellum .
	manualset3
120787	6	404904	5	NULL	NULL	0	NULL	cerebellum 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathological examination revealed the characteristic alterations of spongiform encephalopathy , severe in the thalamus , moderate but widely spread in the cerebral cortices , and moderate in the cerebellum .
	manualset3
120788	1	404905	5	NULL	NULL	0	NULL	Pathology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathology , cause , tests and specific immuno-therapy are presented .
	manualset3
120789	2	404905	5	NULL	NULL	0	NULL	cause 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathology , cause , tests and specific immuno-therapy are presented .
	manualset3
120790	3	404905	5	NULL	NULL	0	NULL	tests 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathology , cause , tests and specific immuno-therapy are presented .
	manualset3
120791	4	404905	5	NULL	NULL	0	NULL	specific immuno-therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathology , cause , tests and specific immuno-therapy are presented .
	manualset3
120792	1	404906	5	NULL	NULL	0	NULL	Pathophysiology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathophysiology of obesity-related hypertension : role of insulin and the sympathetic nervous system .
	manualset3
120793	2	404906	5	NULL	NULL	0	NULL	obesity-related hypertension	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathophysiology of obesity-related hypertension : role of insulin and the sympathetic nervous system .
	manualset3
120794	3	404906	5	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathophysiology of obesity-related hypertension : role of insulin and the sympathetic nervous system .
	manualset3
120795	4	404906	5	NULL	NULL	0	NULL	insulin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathophysiology of obesity-related hypertension : role of insulin and the sympathetic nervous system .
	manualset3
120796	5	404906	5	NULL	NULL	0	NULL	sympathetic nervous system	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathophysiology of obesity-related hypertension : role of insulin and the sympathetic nervous system .
	manualset3
120797	1	404907	5	NULL	NULL	0	NULL	Pathways 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathways mediating cell survival , cell proliferation , and response to stress not only generate signals through various protein kinase pathways to enhance cell survival and proliferation , but these pathways also interact with ERs .
	manualset3
120798	2	404907	5	NULL	NULL	0	NULL	cell survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathways mediating cell survival , cell proliferation , and response to stress not only generate signals through various protein kinase pathways to enhance cell survival and proliferation , but these pathways also interact with ERs .
	manualset3
120799	3	404907	5	NULL	NULL	0	NULL	cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathways mediating cell survival , cell proliferation , and response to stress not only generate signals through various protein kinase pathways to enhance cell survival and proliferation , but these pathways also interact with ERs .
	manualset3
120800	4	404907	5	NULL	NULL	0	NULL	response to stress	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathways mediating cell survival , cell proliferation , and response to stress not only generate signals through various protein kinase pathways to enhance cell survival and proliferation , but these pathways also interact with ERs .
	manualset3
120801	5	404907	5	NULL	NULL	0	NULL	signals 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathways mediating cell survival , cell proliferation , and response to stress not only generate signals through various protein kinase pathways to enhance cell survival and proliferation , but these pathways also interact with ERs .
	manualset3
120802	6	404907	5	NULL	NULL	0	NULL	protein kinase pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathways mediating cell survival , cell proliferation , and response to stress not only generate signals through various protein kinase pathways to enhance cell survival and proliferation , but these pathways also interact with ERs .
	manualset3
120804	8	404907	5	NULL	NULL	0	NULL	cell survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathways mediating cell survival , cell proliferation , and response to stress not only generate signals through various protein kinase pathways to enhance cell survival and proliferation , but these pathways also interact with ERs .
	manualset3
120805	9	404907	5	NULL	NULL	0	NULL	proliferation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathways mediating cell survival , cell proliferation , and response to stress not only generate signals through various protein kinase pathways to enhance cell survival and proliferation , but these pathways also interact with ERs .
	manualset3
120806	10	404907	5	NULL	NULL	0	NULL	pathways 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathways mediating cell survival , cell proliferation , and response to stress not only generate signals through various protein kinase pathways to enhance cell survival and proliferation , but these pathways also interact with ERs .
	manualset3
120807	11	404907	5	NULL	NULL	0	NULL	interact 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathways mediating cell survival , cell proliferation , and response to stress not only generate signals through various protein kinase pathways to enhance cell survival and proliferation , but these pathways also interact with ERs .
	manualset3
120808	12	404907	5	NULL	NULL	NULL	NULL	ERs 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pathways mediating cell survival , cell proliferation , and response to stress not only generate signals through various protein kinase pathways to enhance cell survival and proliferation , but these pathways also interact with ERs .
	manualset3
120809	1	404908	5	NULL	NULL	0	NULL	Pathways 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathways of intracellular hydrogen transport .
	manualset3
120810	2	404908	5	NULL	NULL	0	NULL	intracellular hydrogen transport 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathways of intracellular hydrogen transport .
	manualset3
120811	1	404909	5	NULL	NULL	0	NULL	Patient-focused care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient-focused care is a philosophy incorporating a set of basic principles with which hospitals and other health care institutions organize and facilitate administration and delivery of the caring continuum .
	manualset3
120812	2	404909	5	NULL	NULL	0	NULL	philosophy 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient-focused care is a philosophy incorporating a set of basic principles with which hospitals and other health care institutions organize and facilitate administration and delivery of the caring continuum .
	manualset3
120813	3	404909	5	NULL	NULL	0	NULL	set 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient-focused care is a philosophy incorporating a set of basic principles with which hospitals and other health care institutions organize and facilitate administration and delivery of the caring continuum .
	manualset3
120814	4	404909	5	NULL	NULL	0	NULL	basic principles	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient-focused care is a philosophy incorporating a set of basic principles with which hospitals and other health care institutions organize and facilitate administration and delivery of the caring continuum .
	manualset3
120815	5	404909	5	NULL	NULL	0	NULL	hospitals 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient-focused care is a philosophy incorporating a set of basic principles with which hospitals and other health care institutions organize and facilitate administration and delivery of the caring continuum .
	manualset3
120816	6	404909	5	NULL	NULL	0	NULL	health care institutions	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient-focused care is a philosophy incorporating a set of basic principles with which hospitals and other health care institutions organize and facilitate administration and delivery of the caring continuum .
	manualset3
120817	7	404909	5	NULL	NULL	NULL	NULL	administration 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patient-focused care is a philosophy incorporating a set of basic principles with which hospitals and other health care institutions organize and facilitate administration and delivery of the caring continuum .
	manualset3
120818	8	404909	5	NULL	NULL	NULL	NULL	delivery 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patient-focused care is a philosophy incorporating a set of basic principles with which hospitals and other health care institutions organize and facilitate administration and delivery of the caring continuum .
	manualset3
120819	9	404909	5	NULL	NULL	0	NULL	caring continuum	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient-focused care is a philosophy incorporating a set of basic principles with which hospitals and other health care institutions organize and facilitate administration and delivery of the caring continuum .
	manualset3
120820	1	404910	5	NULL	NULL	NULL	NULL	Patient attitudes	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patient and family attitudes about schizophrenia : implications for genetic counseling .
	manualset3
120821	2	404910	5	NULL	NULL	0	NULL	family attitudes	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient and family attitudes about schizophrenia : implications for genetic counseling .
	manualset3
120822	3	404910	5	NULL	NULL	0	NULL	schizophrenia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient and family attitudes about schizophrenia : implications for genetic counseling .
	manualset3
120823	4	404910	5	NULL	NULL	0	NULL	implications 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient and family attitudes about schizophrenia : implications for genetic counseling .
	manualset3
120824	5	404910	5	NULL	NULL	0	NULL	genetic counseling 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient and family attitudes about schizophrenia : implications for genetic counseling .
	manualset3
120825	1	404911	5	NULL	NULL	NULL	NULL	Patient response	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patient and parent response to the presence or supposed presence of eye disease is a major factor in handling pediatric ophthalmology patients .
	manualset3
120826	2	404911	5	NULL	NULL	0	NULL	parent response 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient and parent response to the presence or supposed presence of eye disease is a major factor in handling pediatric ophthalmology patients .
	manualset3
120827	3	404911	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient and parent response to the presence or supposed presence of eye disease is a major factor in handling pediatric ophthalmology patients .
	manualset3
120828	4	404911	5	NULL	NULL	0	NULL	supposed presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient and parent response to the presence or supposed presence of eye disease is a major factor in handling pediatric ophthalmology patients .
	manualset3
120829	5	404911	5	NULL	NULL	0	NULL	eye disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient and parent response to the presence or supposed presence of eye disease is a major factor in handling pediatric ophthalmology patients .
	manualset3
120830	6	404911	5	NULL	NULL	0	NULL	major factor 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient and parent response to the presence or supposed presence of eye disease is a major factor in handling pediatric ophthalmology patients .
	manualset3
120831	7	404911	5	NULL	NULL	0	NULL	pediatric ophthalmology patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient and parent response to the presence or supposed presence of eye disease is a major factor in handling pediatric ophthalmology patients .
	manualset3
120832	1	404912	5	NULL	NULL	0	NULL	Patient census	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient census for three meals ( breakfast , lunch , and supper ) was compared with the midnight census , using graphical analysis and analysis of variance .
	manualset3
120833	2	404912	5	NULL	NULL	NULL	NULL	three meals ( breakfast , lunch , and supper ) 	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patient census for three meals ( breakfast , lunch , and supper ) was compared with the midnight census , using graphical analysis and analysis of variance .
	manualset3
120834	3	404912	5	NULL	NULL	0	NULL	midnight census 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient census for three meals ( breakfast , lunch , and supper ) was compared with the midnight census , using graphical analysis and analysis of variance .
	manualset3
120835	4	404912	5	NULL	NULL	0	NULL	graphical analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient census for three meals ( breakfast , lunch , and supper ) was compared with the midnight census , using graphical analysis and analysis of variance .
	manualset3
120836	5	404912	5	NULL	NULL	NULL	NULL	 analysis of variance	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patient census for three meals ( breakfast , lunch , and supper ) was compared with the midnight census , using graphical analysis and analysis of variance .
	manualset3
120837	1	404913	5	NULL	NULL	0	NULL	Patient confidentiality	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient confidentiality and consent to publication .
	manualset3
120838	2	404913	5	NULL	NULL	0	NULL	consent 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient confidentiality and consent to publication .
	manualset3
120839	3	404913	5	NULL	NULL	0	NULL	publication 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient confidentiality and consent to publication .
	manualset3
120840	1	404914	5	NULL	NULL	0	NULL	Patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient controlled sedation using a standard protocol for dressing changes in burns : Patients ' preference , procedural details and a preliminary safety evaluation .
	manualset3
120841	2	404914	5	NULL	NULL	0	NULL	sedation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient controlled sedation using a standard protocol for dressing changes in burns : Patients ' preference , procedural details and a preliminary safety evaluation .
	manualset3
120842	3	404914	5	NULL	NULL	0	NULL	standard protocol	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient controlled sedation using a standard protocol for dressing changes in burns : Patients ' preference , procedural details and a preliminary safety evaluation .
	manualset3
120843	4	404914	5	NULL	NULL	0	NULL	dressing changes	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient controlled sedation using a standard protocol for dressing changes in burns : Patients ' preference , procedural details and a preliminary safety evaluation .
	manualset3
120844	5	404914	5	NULL	NULL	0	NULL	burns 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient controlled sedation using a standard protocol for dressing changes in burns : Patients ' preference , procedural details and a preliminary safety evaluation .
	manualset3
120845	6	404914	5	NULL	NULL	0	NULL	Patients ' preference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient controlled sedation using a standard protocol for dressing changes in burns : Patients ' preference , procedural details and a preliminary safety evaluation .
	manualset3
120846	7	404914	5	NULL	NULL	NULL	NULL	procedural details 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patient controlled sedation using a standard protocol for dressing changes in burns : Patients ' preference , procedural details and a preliminary safety evaluation .
	manualset3
120847	8	404914	5	NULL	NULL	0	NULL	preliminary safety evaluation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient controlled sedation using a standard protocol for dressing changes in burns : Patients ' preference , procedural details and a preliminary safety evaluation .
	manualset3
120848	1	404915	5	NULL	NULL	0	NULL	Patient survival rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient survival rates at 1 , 3 , and 5 years were 98 % , 98 % , and 98 % , respectively , for LD , and 95 % , 94 % , and 94 % for CD .
	manualset3
120849	2	404915	5	NULL	NULL	0	NULL	1 year	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient survival rates at 1 , 3 , and 5 years were 98 % , 98 % , and 98 % , respectively , for LD , and 95 % , 94 % , and 94 % for CD .
	manualset3
120850	3	404915	5	NULL	NULL	0	NULL	3 years	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient survival rates at 1 , 3 , and 5 years were 98 % , 98 % , and 98 % , respectively , for LD , and 95 % , 94 % , and 94 % for CD .
	manualset3
120851	4	404915	5	NULL	NULL	0	NULL	5 years	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient survival rates at 1 , 3 , and 5 years were 98 % , 98 % , and 98 % , respectively , for LD , and 95 % , 94 % , and 94 % for CD .
	manualset3
120852	5	404915	5	NULL	NULL	0	NULL	98 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient survival rates at 1 , 3 , and 5 years were 98 % , 98 % , and 98 % , respectively , for LD , and 95 % , 94 % , and 94 % for CD .
	manualset3
120853	6	404915	5	NULL	NULL	0	NULL	98 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient survival rates at 1 , 3 , and 5 years were 98 % , 98 % , and 98 % , respectively , for LD , and 95 % , 94 % , and 94 % for CD .
	manualset3
120854	7	404915	5	NULL	NULL	0	NULL	98 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient survival rates at 1 , 3 , and 5 years were 98 % , 98 % , and 98 % , respectively , for LD , and 95 % , 94 % , and 94 % for CD .
	manualset3
120855	8	404915	5	NULL	NULL	0	NULL	LD	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient survival rates at 1 , 3 , and 5 years were 98 % , 98 % , and 98 % , respectively , for LD , and 95 % , 94 % , and 94 % for CD .
	manualset3
120856	9	404915	5	NULL	NULL	0	NULL	95 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient survival rates at 1 , 3 , and 5 years were 98 % , 98 % , and 98 % , respectively , for LD , and 95 % , 94 % , and 94 % for CD .
	manualset3
120857	10	404915	5	NULL	NULL	0	NULL	94 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient survival rates at 1 , 3 , and 5 years were 98 % , 98 % , and 98 % , respectively , for LD , and 95 % , 94 % , and 94 % for CD .
	manualset3
120858	11	404915	5	NULL	NULL	0	NULL	94 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient survival rates at 1 , 3 , and 5 years were 98 % , 98 % , and 98 % , respectively , for LD , and 95 % , 94 % , and 94 % for CD .
	manualset3
120859	12	404915	5	NULL	NULL	0	NULL	CD 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient survival rates at 1 , 3 , and 5 years were 98 % , 98 % , and 98 % , respectively , for LD , and 95 % , 94 % , and 94 % for CD .
	manualset3
120860	1	404916	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients and their relatives were fully informed of the diagnosis and treatments ( types , risks , practical details ) , but disease progression with and without treatment , like the prognosis , was rarely addressed .
	manualset3
120861	2	404916	5	NULL	NULL	0	NULL	relatives 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients and their relatives were fully informed of the diagnosis and treatments ( types , risks , practical details ) , but disease progression with and without treatment , like the prognosis , was rarely addressed .
	manualset3
120862	3	404916	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients and their relatives were fully informed of the diagnosis and treatments ( types , risks , practical details ) , but disease progression with and without treatment , like the prognosis , was rarely addressed .
	manualset3
120863	4	404916	5	NULL	NULL	0	NULL	treatments 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients and their relatives were fully informed of the diagnosis and treatments ( types , risks , practical details ) , but disease progression with and without treatment , like the prognosis , was rarely addressed .
	manualset3
120864	5	404916	5	NULL	NULL	0	NULL	types 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients and their relatives were fully informed of the diagnosis and treatments ( types , risks , practical details ) , but disease progression with and without treatment , like the prognosis , was rarely addressed .
	manualset3
120865	6	404916	5	NULL	NULL	0	NULL	risks 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients and their relatives were fully informed of the diagnosis and treatments ( types , risks , practical details ) , but disease progression with and without treatment , like the prognosis , was rarely addressed .
	manualset3
120866	7	404916	5	NULL	NULL	0	NULL	practical details	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients and their relatives were fully informed of the diagnosis and treatments ( types , risks , practical details ) , but disease progression with and without treatment , like the prognosis , was rarely addressed .
	manualset3
120867	8	404916	5	NULL	NULL	0	NULL	disease progression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients and their relatives were fully informed of the diagnosis and treatments ( types , risks , practical details ) , but disease progression with and without treatment , like the prognosis , was rarely addressed .
	manualset3
120868	9	404916	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients and their relatives were fully informed of the diagnosis and treatments ( types , risks , practical details ) , but disease progression with and without treatment , like the prognosis , was rarely addressed .
	manualset3
120869	10	404916	5	NULL	NULL	0	NULL	prognosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients and their relatives were fully informed of the diagnosis and treatments ( types , risks , practical details ) , but disease progression with and without treatment , like the prognosis , was rarely addressed .
	manualset3
120870	1	404917	5	NULL	NULL	0	NULL	Patients ' knowledge 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients ' knowledge concerning high blood pressure ( HBP ) is a useful outcome measure in HBP education programs .
	manualset3
120871	2	404917	5	NULL	NULL	0	NULL	high blood pressure ( HBP )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients ' knowledge concerning high blood pressure ( HBP ) is a useful outcome measure in HBP education programs .
	manualset3
120872	3	404917	5	NULL	NULL	NULL	NULL	useful outcome measure	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patients ' knowledge concerning high blood pressure ( HBP ) is a useful outcome measure in HBP education programs .
	manualset3
120873	4	404917	5	NULL	NULL	0	NULL	HBP education programs	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients ' knowledge concerning high blood pressure ( HBP ) is a useful outcome measure in HBP education programs .
	manualset3
120874	1	404918	5	NULL	NULL	0	NULL	general kinetic approach 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A general kinetic approach was adopted to interpret the dependence of the applied potential upon the scan rate at constant pH and upon pH at constant scan rate , while keeping the initial reactant concentration and the faradaic charge constant .
	manualset3
120875	2	404918	5	NULL	NULL	0	NULL	dependence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A general kinetic approach was adopted to interpret the dependence of the applied potential upon the scan rate at constant pH and upon pH at constant scan rate , while keeping the initial reactant concentration and the faradaic charge constant .
	manualset3
120876	3	404918	5	NULL	NULL	0	NULL	applied potential 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A general kinetic approach was adopted to interpret the dependence of the applied potential upon the scan rate at constant pH and upon pH at constant scan rate , while keeping the initial reactant concentration and the faradaic charge constant .
	manualset3
120877	4	404918	5	NULL	NULL	0	NULL	scan rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A general kinetic approach was adopted to interpret the dependence of the applied potential upon the scan rate at constant pH and upon pH at constant scan rate , while keeping the initial reactant concentration and the faradaic charge constant .
	manualset3
120878	5	404918	5	NULL	NULL	0	NULL	constant pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A general kinetic approach was adopted to interpret the dependence of the applied potential upon the scan rate at constant pH and upon pH at constant scan rate , while keeping the initial reactant concentration and the faradaic charge constant .
	manualset3
120879	6	404918	5	NULL	NULL	0	NULL	pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A general kinetic approach was adopted to interpret the dependence of the applied potential upon the scan rate at constant pH and upon pH at constant scan rate , while keeping the initial reactant concentration and the faradaic charge constant .
	manualset3
120880	7	404918	5	NULL	NULL	0	NULL	constant scan rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A general kinetic approach was adopted to interpret the dependence of the applied potential upon the scan rate at constant pH and upon pH at constant scan rate , while keeping the initial reactant concentration and the faradaic charge constant .
	manualset3
120881	8	404918	5	NULL	NULL	0	NULL	initial reactant concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A general kinetic approach was adopted to interpret the dependence of the applied potential upon the scan rate at constant pH and upon pH at constant scan rate , while keeping the initial reactant concentration and the faradaic charge constant .
	manualset3
120882	9	404918	5	NULL	NULL	0	NULL	faradaic charge constant	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A general kinetic approach was adopted to interpret the dependence of the applied potential upon the scan rate at constant pH and upon pH at constant scan rate , while keeping the initial reactant concentration and the faradaic charge constant .
	manualset3
120883	1	404919	5	NULL	NULL	NULL	NULL	faradaic charge constant	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patients ( n = 104 ) visiting the university clinic ( UC ) of the Academic Centre for Dentistry Amsterdam ( ACTA ) , were interviewed during their first visit .
	manualset3
120884	2	404919	5	NULL	NULL	0	NULL	n = 104 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients ( n = 104 ) visiting the university clinic ( UC ) of the Academic Centre for Dentistry Amsterdam ( ACTA ) , were interviewed during their first visit .
	manualset3
120885	3	404919	5	NULL	NULL	0	NULL	university clinic ( UC ) 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients ( n = 104 ) visiting the university clinic ( UC ) of the Academic Centre for Dentistry Amsterdam ( ACTA ) , were interviewed during their first visit .
	manualset3
120886	4	404919	5	NULL	NULL	0	NULL	Academic Centre for Dentistry Amsterdam ( ACTA ) 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients ( n = 104 ) visiting the university clinic ( UC ) of the Academic Centre for Dentistry Amsterdam ( ACTA ) , were interviewed during their first visit .
	manualset3
120887	5	404919	5	NULL	NULL	0	NULL	first visit 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients ( n = 104 ) visiting the university clinic ( UC ) of the Academic Centre for Dentistry Amsterdam ( ACTA ) , were interviewed during their first visit .
	manualset3
120888	1	404920	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients attending a dedicated dental clinic during the previous 24 months were assessed for the success of root canal treatment .
	manualset3
120889	2	404920	5	NULL	NULL	0	NULL	dedicated dental clinic 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients attending a dedicated dental clinic during the previous 24 months were assessed for the success of root canal treatment .
	manualset3
120890	3	404920	5	NULL	NULL	0	NULL	previous 24 months 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients attending a dedicated dental clinic during the previous 24 months were assessed for the success of root canal treatment .
	manualset3
120891	4	404920	5	NULL	NULL	0	NULL	success 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients attending a dedicated dental clinic during the previous 24 months were assessed for the success of root canal treatment .
	manualset3
120892	5	404920	5	NULL	NULL	0	NULL	root canal treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients attending a dedicated dental clinic during the previous 24 months were assessed for the success of root canal treatment .
	manualset3
120893	1	404921	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients had metabolic shifts toward increased production of monounsaturated fatty acids and increased ratios of derivatives to precursors of omega 6 fatty acids , shifts that occur when cells are EFA-deficient .
	manualset3
120894	2	404921	5	NULL	NULL	0	NULL	metabolic shifts 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients had metabolic shifts toward increased production of monounsaturated fatty acids and increased ratios of derivatives to precursors of omega 6 fatty acids , shifts that occur when cells are EFA-deficient .
	manualset3
120895	3	404921	5	NULL	NULL	0	NULL	increased production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients had metabolic shifts toward increased production of monounsaturated fatty acids and increased ratios of derivatives to precursors of omega 6 fatty acids , shifts that occur when cells are EFA-deficient .
	manualset3
120896	4	404921	5	NULL	NULL	0	NULL	monounsaturated fatty acids 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients had metabolic shifts toward increased production of monounsaturated fatty acids and increased ratios of derivatives to precursors of omega 6 fatty acids , shifts that occur when cells are EFA-deficient .
	manualset3
120897	5	404921	5	NULL	NULL	0	NULL	increased ratios	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients had metabolic shifts toward increased production of monounsaturated fatty acids and increased ratios of derivatives to precursors of omega 6 fatty acids , shifts that occur when cells are EFA-deficient .
	manualset3
120898	6	404921	5	NULL	NULL	0	NULL	derivatives 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients had metabolic shifts toward increased production of monounsaturated fatty acids and increased ratios of derivatives to precursors of omega 6 fatty acids , shifts that occur when cells are EFA-deficient .
	manualset3
120899	7	404921	5	NULL	NULL	0	NULL	precursors of omega 6 fatty acids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients had metabolic shifts toward increased production of monounsaturated fatty acids and increased ratios of derivatives to precursors of omega 6 fatty acids , shifts that occur when cells are EFA-deficient .
	manualset3
120900	8	404921	5	NULL	NULL	0	NULL	shifts 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients had metabolic shifts toward increased production of monounsaturated fatty acids and increased ratios of derivatives to precursors of omega 6 fatty acids , shifts that occur when cells are EFA-deficient .
	manualset3
120901	9	404921	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients had metabolic shifts toward increased production of monounsaturated fatty acids and increased ratios of derivatives to precursors of omega 6 fatty acids , shifts that occur when cells are EFA-deficient .
	manualset3
120902	1	404922	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients handed the completed questionnaires to their practitioner , who indicated the type of visit and the focus of the encounter .
	manualset3
120903	2	404922	5	NULL	NULL	0	NULL	completed questionnaires 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients handed the completed questionnaires to their practitioner , who indicated the type of visit and the focus of the encounter .
	manualset3
120904	3	404922	5	NULL	NULL	0	NULL	practitioner 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients handed the completed questionnaires to their practitioner , who indicated the type of visit and the focus of the encounter .
	manualset3
120905	4	404922	5	NULL	NULL	NULL	NULL	type 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patients handed the completed questionnaires to their practitioner , who indicated the type of visit and the focus of the encounter .
	manualset3
120906	5	404922	5	NULL	NULL	0	NULL	visit 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients handed the completed questionnaires to their practitioner , who indicated the type of visit and the focus of the encounter .
	manualset3
120907	6	404922	5	NULL	NULL	0	NULL	focus 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients handed the completed questionnaires to their practitioner , who indicated the type of visit and the focus of the encounter .
	manualset3
120908	7	404922	5	NULL	NULL	0	NULL	encounter 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients handed the completed questionnaires to their practitioner , who indicated the type of visit and the focus of the encounter .
	manualset3
120909	1	404923	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients harboring circulating prostatic tumor cells as detected by prostate specific membrane and not by PSA polymerase chain reaction included 7 of 13 previously treated by radical prostatectomy who had nonmeasurable serum PSA levels at the time of this assay .
	manualset3
120910	2	404923	5	NULL	NULL	0	NULL	circulating prostatic tumor cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients harboring circulating prostatic tumor cells as detected by prostate specific membrane and not by PSA polymerase chain reaction included 7 of 13 previously treated by radical prostatectomy who had nonmeasurable serum PSA levels at the time of this assay .
	manualset3
120911	3	404923	5	NULL	NULL	0	NULL	prostate specific membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients harboring circulating prostatic tumor cells as detected by prostate specific membrane and not by PSA polymerase chain reaction included 7 of 13 previously treated by radical prostatectomy who had nonmeasurable serum PSA levels at the time of this assay .
	manualset3
120912	4	404923	5	NULL	NULL	0	NULL	PSA polymerase chain reaction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients harboring circulating prostatic tumor cells as detected by prostate specific membrane and not by PSA polymerase chain reaction included 7 of 13 previously treated by radical prostatectomy who had nonmeasurable serum PSA levels at the time of this assay .
	manualset3
120913	5	404923	5	NULL	NULL	0	NULL	7 of 13	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients harboring circulating prostatic tumor cells as detected by prostate specific membrane and not by PSA polymerase chain reaction included 7 of 13 previously treated by radical prostatectomy who had nonmeasurable serum PSA levels at the time of this assay .
	manualset3
120914	6	404923	5	NULL	NULL	0	NULL	radical prostatectomy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients harboring circulating prostatic tumor cells as detected by prostate specific membrane and not by PSA polymerase chain reaction included 7 of 13 previously treated by radical prostatectomy who had nonmeasurable serum PSA levels at the time of this assay .
	manualset3
120915	7	404923	5	NULL	NULL	0	NULL	nonmeasurable serum PSA levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients harboring circulating prostatic tumor cells as detected by prostate specific membrane and not by PSA polymerase chain reaction included 7 of 13 previously treated by radical prostatectomy who had nonmeasurable serum PSA levels at the time of this assay .
	manualset3
120916	8	404923	5	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients harboring circulating prostatic tumor cells as detected by prostate specific membrane and not by PSA polymerase chain reaction included 7 of 13 previously treated by radical prostatectomy who had nonmeasurable serum PSA levels at the time of this assay .
	manualset3
120917	9	404923	5	NULL	NULL	0	NULL	assay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients harboring circulating prostatic tumor cells as detected by prostate specific membrane and not by PSA polymerase chain reaction included 7 of 13 previously treated by radical prostatectomy who had nonmeasurable serum PSA levels at the time of this assay .
	manualset3
120918	1	404924	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in II radiological stage shower higher PIIIP concentrations in BALF than patients in I stage of sarcoidosis .
	manualset3
120919	2	404924	5	NULL	NULL	0	NULL	II radiological stage	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in II radiological stage shower higher PIIIP concentrations in BALF than patients in I stage of sarcoidosis .
	manualset3
120920	3	404924	5	NULL	NULL	0	NULL	PIIIP concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in II radiological stage shower higher PIIIP concentrations in BALF than patients in I stage of sarcoidosis .
	manualset3
120921	4	404924	5	NULL	NULL	0	NULL	BALF	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in II radiological stage shower higher PIIIP concentrations in BALF than patients in I stage of sarcoidosis .
	manualset3
120922	5	404924	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in II radiological stage shower higher PIIIP concentrations in BALF than patients in I stage of sarcoidosis .
	manualset3
120923	6	404924	5	NULL	NULL	0	NULL	I stage 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in II radiological stage shower higher PIIIP concentrations in BALF than patients in I stage of sarcoidosis .
	manualset3
120924	7	404924	5	NULL	NULL	0	NULL	sarcoidosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in II radiological stage shower higher PIIIP concentrations in BALF than patients in I stage of sarcoidosis .
	manualset3
120925	1	404925	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in early clinical stage ( Binet A , Rai 0 ) with non-diffuse bone marrow histopathology , and low , stable blood lymphocyte levels have a long survival and should not be treated unless the disease progresses .
	manualset3
120926	2	404925	5	NULL	NULL	NULL	NULL	early clinical stage ( Binet A , Rai 0 ) 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patients in early clinical stage ( Binet A , Rai 0 ) with non-diffuse bone marrow histopathology , and low , stable blood lymphocyte levels have a long survival and should not be treated unless the disease progresses .
	manualset3
120927	3	404925	5	NULL	NULL	0	NULL	non-diffuse bone marrow histopathology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in early clinical stage ( Binet A , Rai 0 ) with non-diffuse bone marrow histopathology , and low , stable blood lymphocyte levels have a long survival and should not be treated unless the disease progresses .
	manualset3
120928	4	404925	5	NULL	NULL	0	NULL	low , stable blood lymphocyte levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in early clinical stage ( Binet A , Rai 0 ) with non-diffuse bone marrow histopathology , and low , stable blood lymphocyte levels have a long survival and should not be treated unless the disease progresses .
	manualset3
120929	5	404925	5	NULL	NULL	0	NULL	survival 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in early clinical stage ( Binet A , Rai 0 ) with non-diffuse bone marrow histopathology , and low , stable blood lymphocyte levels have a long survival and should not be treated unless the disease progresses .
	manualset3
120930	6	404925	5	NULL	NULL	0	NULL	disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in early clinical stage ( Binet A , Rai 0 ) with non-diffuse bone marrow histopathology , and low , stable blood lymphocyte levels have a long survival and should not be treated unless the disease progresses .
	manualset3
120931	1	404926	5	NULL	NULL	0	NULL	general method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A general method for the Suzuki-Miyaura cross-coupling of sterically hindered aryl chlorides : synthesis of di - and tri-ortho-substituted biaryls in 2-propanol at room temperature .
	manualset3
120932	2	404926	5	NULL	NULL	0	NULL	Suzuki-Miyaura cross-coupling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A general method for the Suzuki-Miyaura cross-coupling of sterically hindered aryl chlorides : synthesis of di - and tri-ortho-substituted biaryls in 2-propanol at room temperature .
	manualset3
120933	3	404926	5	NULL	NULL	0	NULL	sterically hindered aryl chlorides 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A general method for the Suzuki-Miyaura cross-coupling of sterically hindered aryl chlorides : synthesis of di - and tri-ortho-substituted biaryls in 2-propanol at room temperature .
	manualset3
120934	4	404926	5	NULL	NULL	0	NULL	di - and tri-ortho-substituted biaryls 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A general method for the Suzuki-Miyaura cross-coupling of sterically hindered aryl chlorides : synthesis of di - and tri-ortho-substituted biaryls in 2-propanol at room temperature .
	manualset3
120935	5	404926	5	NULL	NULL	0	NULL	2-propanol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A general method for the Suzuki-Miyaura cross-coupling of sterically hindered aryl chlorides : synthesis of di - and tri-ortho-substituted biaryls in 2-propanol at room temperature .
	manualset3
120936	6	404926	5	NULL	NULL	0	NULL	room temperature	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A general method for the Suzuki-Miyaura cross-coupling of sterically hindered aryl chlorides : synthesis of di - and tri-ortho-substituted biaryls in 2-propanol at room temperature .
	manualset3
120937	1	404927	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in group 2 showed a reduction in plasma LDL-C levels of 35 % and in LDL-C to high-density lipoprotein cholesterol ( HDL-C ) ratio of 45 % compared with 32 % and 38 % respectively in group 1 .
	manualset3
120938	2	404927	5	NULL	NULL	0	NULL	group 2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in group 2 showed a reduction in plasma LDL-C levels of 35 % and in LDL-C to high-density lipoprotein cholesterol ( HDL-C ) ratio of 45 % compared with 32 % and 38 % respectively in group 1 .
	manualset3
120939	3	404927	5	NULL	NULL	0	NULL	reduction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in group 2 showed a reduction in plasma LDL-C levels of 35 % and in LDL-C to high-density lipoprotein cholesterol ( HDL-C ) ratio of 45 % compared with 32 % and 38 % respectively in group 1 .
	manualset3
120940	4	404927	5	NULL	NULL	0	NULL	plasma LDL-C levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in group 2 showed a reduction in plasma LDL-C levels of 35 % and in LDL-C to high-density lipoprotein cholesterol ( HDL-C ) ratio of 45 % compared with 32 % and 38 % respectively in group 1 .
	manualset3
120941	5	404927	5	NULL	NULL	0	NULL	35 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in group 2 showed a reduction in plasma LDL-C levels of 35 % and in LDL-C to high-density lipoprotein cholesterol ( HDL-C ) ratio of 45 % compared with 32 % and 38 % respectively in group 1 .
	manualset3
120942	6	404927	5	NULL	NULL	NULL	NULL	 LDL-C to high-density lipoprotein cholesterol ( HDL-C ) ratio 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patients in group 2 showed a reduction in plasma LDL-C levels of 35 % and in LDL-C to high-density lipoprotein cholesterol ( HDL-C ) ratio of 45 % compared with 32 % and 38 % respectively in group 1 .
	manualset3
120943	7	404927	5	NULL	NULL	NULL	NULL	45 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patients in group 2 showed a reduction in plasma LDL-C levels of 35 % and in LDL-C to high-density lipoprotein cholesterol ( HDL-C ) ratio of 45 % compared with 32 % and 38 % respectively in group 1 .
	manualset3
120944	8	404927	5	NULL	NULL	0	NULL	32 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in group 2 showed a reduction in plasma LDL-C levels of 35 % and in LDL-C to high-density lipoprotein cholesterol ( HDL-C ) ratio of 45 % compared with 32 % and 38 % respectively in group 1 .
	manualset3
120945	9	404927	5	NULL	NULL	0	NULL	38 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in group 2 showed a reduction in plasma LDL-C levels of 35 % and in LDL-C to high-density lipoprotein cholesterol ( HDL-C ) ratio of 45 % compared with 32 % and 38 % respectively in group 1 .
	manualset3
120946	10	404927	5	NULL	NULL	0	NULL	 group 1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in group 2 showed a reduction in plasma LDL-C levels of 35 % and in LDL-C to high-density lipoprotein cholesterol ( HDL-C ) ratio of 45 % compared with 32 % and 38 % respectively in group 1 .
	manualset3
120947	1	404928	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in group B received cetrizine 10 mg daily and placebo tablets twice daily .
	manualset3
120948	2	404928	5	NULL	NULL	0	NULL	group B	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in group B received cetrizine 10 mg daily and placebo tablets twice daily .
	manualset3
120949	3	404928	5	NULL	NULL	0	NULL	cetrizine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in group B received cetrizine 10 mg daily and placebo tablets twice daily .
	manualset3
120950	4	404928	5	NULL	NULL	0	NULL	10 mg daily 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in group B received cetrizine 10 mg daily and placebo tablets twice daily .
	manualset3
120951	5	404928	5	NULL	NULL	0	NULL	placebo tablets	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in group B received cetrizine 10 mg daily and placebo tablets twice daily .
	manualset3
120952	6	404928	5	NULL	NULL	0	NULL	twice daily 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in group B received cetrizine 10 mg daily and placebo tablets twice daily .
	manualset3
120953	1	404929	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in the low 5-HIAA mode ( below 15 ng/ml ) attempted suicide significantly more often than those in the high mode , and they used more violent means .
	manualset3
120954	2	404929	5	NULL	NULL	0	NULL	low 5-HIAA mode	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in the low 5-HIAA mode ( below 15 ng/ml ) attempted suicide significantly more often than those in the high mode , and they used more violent means .
	manualset3
120955	3	404929	5	NULL	NULL	0	NULL	15 ng/ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in the low 5-HIAA mode ( below 15 ng/ml ) attempted suicide significantly more often than those in the high mode , and they used more violent means .
	manualset3
120956	4	404929	5	NULL	NULL	0	NULL	suicide 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in the low 5-HIAA mode ( below 15 ng/ml ) attempted suicide significantly more often than those in the high mode , and they used more violent means .
	manualset3
120957	5	404929	5	NULL	NULL	0	NULL	 high mode	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in the low 5-HIAA mode ( below 15 ng/ml ) attempted suicide significantly more often than those in the high mode , and they used more violent means .
	manualset3
120958	6	404929	5	NULL	NULL	0	NULL	violent means 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in the low 5-HIAA mode ( below 15 ng/ml ) attempted suicide significantly more often than those in the high mode , and they used more violent means .
	manualset3
120959	1	404930	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients initially were given infusions of decadron followed by macroaggregated albumin and 30 mCi colloidal 32P to the interstitial space of the tumor by two infusions 1 week apart .
	manualset3
120960	2	404930	5	NULL	NULL	0	NULL	infusions 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients initially were given infusions of decadron followed by macroaggregated albumin and 30 mCi colloidal 32P to the interstitial space of the tumor by two infusions 1 week apart .
	manualset3
120961	3	404930	5	NULL	NULL	0	NULL	decadron 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients initially were given infusions of decadron followed by macroaggregated albumin and 30 mCi colloidal 32P to the interstitial space of the tumor by two infusions 1 week apart .
	manualset3
120962	4	404930	5	NULL	NULL	NULL	NULL	macroaggregated albumin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patients initially were given infusions of decadron followed by macroaggregated albumin and 30 mCi colloidal 32P to the interstitial space of the tumor by two infusions 1 week apart .
	manualset3
120963	5	404930	5	NULL	NULL	0	NULL	30 mCi colloidal 32P	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients initially were given infusions of decadron followed by macroaggregated albumin and 30 mCi colloidal 32P to the interstitial space of the tumor by two infusions 1 week apart .
	manualset3
120964	6	404930	5	NULL	NULL	0	NULL	interstitial space	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients initially were given infusions of decadron followed by macroaggregated albumin and 30 mCi colloidal 32P to the interstitial space of the tumor by two infusions 1 week apart .
	manualset3
120965	7	404930	5	NULL	NULL	0	NULL	tumor 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients initially were given infusions of decadron followed by macroaggregated albumin and 30 mCi colloidal 32P to the interstitial space of the tumor by two infusions 1 week apart .
	manualset3
120966	8	404930	5	NULL	NULL	0	NULL	two infusions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients initially were given infusions of decadron followed by macroaggregated albumin and 30 mCi colloidal 32P to the interstitial space of the tumor by two infusions 1 week apart .
	manualset3
120967	9	404930	5	NULL	NULL	0	NULL	1 week 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients initially were given infusions of decadron followed by macroaggregated albumin and 30 mCi colloidal 32P to the interstitial space of the tumor by two infusions 1 week apart .
	manualset3
121308	1	404931	5	NULL	NULL	0	NULL	Patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients negative for class III beta-tubulin expression had a significantly longer median progression-free ( 40 weeks vs. 35 weeks , P = 0.031 ) , but not overall ( 78 weeks vs. 57 weeks , P = 0.087 ) , survival than those positive for class III beta-tubulin expression .
	manualset3
121309	2	404931	5	NULL	NULL	0	NULL	class III beta-tubulin expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients negative for class III beta-tubulin expression had a significantly longer median progression-free ( 40 weeks vs. 35 weeks , P = 0.031 ) , but not overall ( 78 weeks vs. 57 weeks , P = 0.087 ) , survival than those positive for class III beta-tubulin expression .
	manualset3
121319	3	404931	5	NULL	NULL	0	NULL	 longer median progression-free survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients negative for class III beta-tubulin expression had a significantly longer median progression-free ( 40 weeks vs. 35 weeks , P = 0.031 ) , but not overall ( 78 weeks vs. 57 weeks , P = 0.087 ) , survival than those positive for class III beta-tubulin expression .
	manualset3
121321	4	404931	5	NULL	NULL	0	NULL	40 weeks vs. 35 weeks , P = 0.031	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients negative for class III beta-tubulin expression had a significantly longer median progression-free ( 40 weeks vs. 35 weeks , P = 0.031 ) , but not overall ( 78 weeks vs. 57 weeks , P = 0.087 ) , survival than those positive for class III beta-tubulin expression .
	manualset3
121323	5	404931	5	NULL	NULL	0	NULL	78 weeks vs. 57 weeks , P = 0.087	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients negative for class III beta-tubulin expression had a significantly longer median progression-free ( 40 weeks vs. 35 weeks , P = 0.031 ) , but not overall ( 78 weeks vs. 57 weeks , P = 0.087 ) , survival than those positive for class III beta-tubulin expression .
	manualset3
121324	6	404931	5	NULL	NULL	0	NULL	overall survival 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients negative for class III beta-tubulin expression had a significantly longer median progression-free ( 40 weeks vs. 35 weeks , P = 0.031 ) , but not overall ( 78 weeks vs. 57 weeks , P = 0.087 ) , survival than those positive for class III beta-tubulin expression .
	manualset3
121325	7	404931	5	NULL	NULL	0	NULL	class III beta-tubulin expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients negative for class III beta-tubulin expression had a significantly longer median progression-free ( 40 weeks vs. 35 weeks , P = 0.031 ) , but not overall ( 78 weeks vs. 57 weeks , P = 0.087 ) , survival than those positive for class III beta-tubulin expression .
	manualset3
121326	1	404932	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients of the PCEA group received 3 ml of 0.1 % bupivacaine plus 2 microg/ml of fentanyl per demand , with continuous background infusion of 6ml/h .
	manualset3
121327	2	404932	5	NULL	NULL	0	NULL	PCEA group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients of the PCEA group received 3 ml of 0.1 % bupivacaine plus 2 microg/ml of fentanyl per demand , with continuous background infusion of 6ml/h .
	manualset3
121328	3	404932	5	NULL	NULL	0	NULL	3 ml of 0.1 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients of the PCEA group received 3 ml of 0.1 % bupivacaine plus 2 microg/ml of fentanyl per demand , with continuous background infusion of 6ml/h .
	manualset3
121329	4	404932	5	NULL	NULL	0	NULL	bupivacaine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients of the PCEA group received 3 ml of 0.1 % bupivacaine plus 2 microg/ml of fentanyl per demand , with continuous background infusion of 6ml/h .
	manualset3
121330	5	404932	5	NULL	NULL	0	NULL	2 microg/ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients of the PCEA group received 3 ml of 0.1 % bupivacaine plus 2 microg/ml of fentanyl per demand , with continuous background infusion of 6ml/h .
	manualset3
121331	6	404932	5	NULL	NULL	0	NULL	fentanyl 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients of the PCEA group received 3 ml of 0.1 % bupivacaine plus 2 microg/ml of fentanyl per demand , with continuous background infusion of 6ml/h .
	manualset3
121332	7	404932	5	NULL	NULL	0	NULL	demand 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients of the PCEA group received 3 ml of 0.1 % bupivacaine plus 2 microg/ml of fentanyl per demand , with continuous background infusion of 6ml/h .
	manualset3
121495	8	404932	5	NULL	NULL	0	NULL	continuous background infusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients of the PCEA group received 3 ml of 0.1 % bupivacaine plus 2 microg/ml of fentanyl per demand , with continuous background infusion of 6ml/h .
	manualset3
121496	9	404932	5	NULL	NULL	0	NULL	6ml/h	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients of the PCEA group received 3 ml of 0.1 % bupivacaine plus 2 microg/ml of fentanyl per demand , with continuous background infusion of 6ml/h .
	manualset3
121497	1	404933	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients received a total oral busulfan dose of 11 to 28 mg/kg followed by a total cyclophosphamide dose of 120 to 335 mg/kg in preparation for allogeneic grafts ( HLA-matched or HLA partially matched sibling , parent or unrelated donor ) .
	manualset3
121498	2	404933	5	NULL	NULL	0	NULL	total oral busulfan dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients received a total oral busulfan dose of 11 to 28 mg/kg followed by a total cyclophosphamide dose of 120 to 335 mg/kg in preparation for allogeneic grafts ( HLA-matched or HLA partially matched sibling , parent or unrelated donor ) .
	manualset3
121499	3	404933	5	NULL	NULL	0	NULL	11 to 28 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients received a total oral busulfan dose of 11 to 28 mg/kg followed by a total cyclophosphamide dose of 120 to 335 mg/kg in preparation for allogeneic grafts ( HLA-matched or HLA partially matched sibling , parent or unrelated donor ) .
	manualset3
121500	4	404933	5	NULL	NULL	0	NULL	total cyclophosphamide dose 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients received a total oral busulfan dose of 11 to 28 mg/kg followed by a total cyclophosphamide dose of 120 to 335 mg/kg in preparation for allogeneic grafts ( HLA-matched or HLA partially matched sibling , parent or unrelated donor ) .
	manualset3
121501	5	404933	5	NULL	NULL	0	NULL	120 to 335 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients received a total oral busulfan dose of 11 to 28 mg/kg followed by a total cyclophosphamide dose of 120 to 335 mg/kg in preparation for allogeneic grafts ( HLA-matched or HLA partially matched sibling , parent or unrelated donor ) .
	manualset3
121502	6	404933	5	NULL	NULL	0	NULL	preparation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients received a total oral busulfan dose of 11 to 28 mg/kg followed by a total cyclophosphamide dose of 120 to 335 mg/kg in preparation for allogeneic grafts ( HLA-matched or HLA partially matched sibling , parent or unrelated donor ) .
	manualset3
121503	7	404933	5	NULL	NULL	0	NULL	allogeneic grafts	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients received a total oral busulfan dose of 11 to 28 mg/kg followed by a total cyclophosphamide dose of 120 to 335 mg/kg in preparation for allogeneic grafts ( HLA-matched or HLA partially matched sibling , parent or unrelated donor ) .
	manualset3
121504	8	404933	5	NULL	NULL	0	NULL	HLA-matched or HLA partially matched sibling	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients received a total oral busulfan dose of 11 to 28 mg/kg followed by a total cyclophosphamide dose of 120 to 335 mg/kg in preparation for allogeneic grafts ( HLA-matched or HLA partially matched sibling , parent or unrelated donor ) .
	manualset3
121505	9	404933	5	NULL	NULL	0	NULL	HLA-matched or HLA partially matched parent	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients received a total oral busulfan dose of 11 to 28 mg/kg followed by a total cyclophosphamide dose of 120 to 335 mg/kg in preparation for allogeneic grafts ( HLA-matched or HLA partially matched sibling , parent or unrelated donor ) .
	manualset3
121506	10	404933	5	NULL	NULL	0	NULL	HLA-matched or HLA partially matched unrelated donor	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients received a total oral busulfan dose of 11 to 28 mg/kg followed by a total cyclophosphamide dose of 120 to 335 mg/kg in preparation for allogeneic grafts ( HLA-matched or HLA partially matched sibling , parent or unrelated donor ) .
	manualset3
121507	1	404934	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients receiving fVIII/fIX prophylaxis showed a similar trend of increased clot stability in the presence of Solulin .
	manualset3
121508	2	404934	5	NULL	NULL	0	NULL	fVIII/fIX prophylaxis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients receiving fVIII/fIX prophylaxis showed a similar trend of increased clot stability in the presence of Solulin .
	manualset3
121509	3	404934	5	NULL	NULL	0	NULL	trend 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients receiving fVIII/fIX prophylaxis showed a similar trend of increased clot stability in the presence of Solulin .
	manualset3
121510	4	404934	5	NULL	NULL	0	NULL	increased clot stability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients receiving fVIII/fIX prophylaxis showed a similar trend of increased clot stability in the presence of Solulin .
	manualset3
121511	5	404934	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients receiving fVIII/fIX prophylaxis showed a similar trend of increased clot stability in the presence of Solulin .
	manualset3
121512	6	404934	5	NULL	NULL	0	NULL	Solulin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients receiving fVIII/fIX prophylaxis showed a similar trend of increased clot stability in the presence of Solulin .
	manualset3
121513	1	404935	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients receiving tumor necrosis factor alpha inhibitors for the treatment of rheumatic diseases ( rheumatoid arthritis , psoriatic arthritis , ankylosing spondylitis ) are at high risk of developing tuberculosis during treatment .
	manualset3
121514	2	404935	5	NULL	NULL	0	NULL	tumor necrosis factor alpha inhibitors	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients receiving tumor necrosis factor alpha inhibitors for the treatment of rheumatic diseases ( rheumatoid arthritis , psoriatic arthritis , ankylosing spondylitis ) are at high risk of developing tuberculosis during treatment .
	manualset3
121515	3	404935	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients receiving tumor necrosis factor alpha inhibitors for the treatment of rheumatic diseases ( rheumatoid arthritis , psoriatic arthritis , ankylosing spondylitis ) are at high risk of developing tuberculosis during treatment .
	manualset3
121516	4	404935	5	NULL	NULL	0	NULL	rheumatic diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients receiving tumor necrosis factor alpha inhibitors for the treatment of rheumatic diseases ( rheumatoid arthritis , psoriatic arthritis , ankylosing spondylitis ) are at high risk of developing tuberculosis during treatment .
	manualset3
121517	5	404935	5	NULL	NULL	0	NULL	rheumatoid arthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients receiving tumor necrosis factor alpha inhibitors for the treatment of rheumatic diseases ( rheumatoid arthritis , psoriatic arthritis , ankylosing spondylitis ) are at high risk of developing tuberculosis during treatment .
	manualset3
121518	6	404935	5	NULL	NULL	0	NULL	psoriatic arthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients receiving tumor necrosis factor alpha inhibitors for the treatment of rheumatic diseases ( rheumatoid arthritis , psoriatic arthritis , ankylosing spondylitis ) are at high risk of developing tuberculosis during treatment .
	manualset3
121519	7	404935	5	NULL	NULL	0	NULL	ankylosing spondylitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients receiving tumor necrosis factor alpha inhibitors for the treatment of rheumatic diseases ( rheumatoid arthritis , psoriatic arthritis , ankylosing spondylitis ) are at high risk of developing tuberculosis during treatment .
	manualset3
121520	8	404935	5	NULL	NULL	0	NULL	high risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients receiving tumor necrosis factor alpha inhibitors for the treatment of rheumatic diseases ( rheumatoid arthritis , psoriatic arthritis , ankylosing spondylitis ) are at high risk of developing tuberculosis during treatment .
	manualset3
121521	9	404935	5	NULL	NULL	0	NULL	tuberculosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients receiving tumor necrosis factor alpha inhibitors for the treatment of rheumatic diseases ( rheumatoid arthritis , psoriatic arthritis , ankylosing spondylitis ) are at high risk of developing tuberculosis during treatment .
	manualset3
121522	10	404935	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients receiving tumor necrosis factor alpha inhibitors for the treatment of rheumatic diseases ( rheumatoid arthritis , psoriatic arthritis , ankylosing spondylitis ) are at high risk of developing tuberculosis during treatment .
	manualset3
121523	1	404936	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients should be cautioned not to split or crush a medication without checking with the health care provider or pharmacist .
	manualset3
121526	2	404936	5	NULL	NULL	NULL	NULL	medication 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patients should be cautioned not to split or crush a medication without checking with the health care provider or pharmacist .
	manualset3
121527	3	404936	5	NULL	NULL	NULL	NULL	health care provider	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patients should be cautioned not to split or crush a medication without checking with the health care provider or pharmacist .
	manualset3
121528	4	404936	5	NULL	NULL	NULL	NULL	pharmacist 	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patients should be cautioned not to split or crush a medication without checking with the health care provider or pharmacist .
	manualset3
121529	1	404937	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients should have an awareness of their disease , and as health care providers , PD nurses have the role of focusing their patients on preventive care , rather than of simply training patients .
	manualset3
121530	2	404937	5	NULL	NULL	0	NULL	awareness 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients should have an awareness of their disease , and as health care providers , PD nurses have the role of focusing their patients on preventive care , rather than of simply training patients .
	manualset3
121531	3	404937	5	NULL	NULL	0	NULL	disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients should have an awareness of their disease , and as health care providers , PD nurses have the role of focusing their patients on preventive care , rather than of simply training patients .
	manualset3
121532	4	404937	5	NULL	NULL	0	NULL	health care providers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients should have an awareness of their disease , and as health care providers , PD nurses have the role of focusing their patients on preventive care , rather than of simply training patients .
	manualset3
121533	5	404937	5	NULL	NULL	0	NULL	PD nurses	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients should have an awareness of their disease , and as health care providers , PD nurses have the role of focusing their patients on preventive care , rather than of simply training patients .
	manualset3
121534	6	404937	5	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients should have an awareness of their disease , and as health care providers , PD nurses have the role of focusing their patients on preventive care , rather than of simply training patients .
	manualset3
121535	7	404937	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients should have an awareness of their disease , and as health care providers , PD nurses have the role of focusing their patients on preventive care , rather than of simply training patients .
	manualset3
121536	8	404937	5	NULL	NULL	0	NULL	preventive care	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients should have an awareness of their disease , and as health care providers , PD nurses have the role of focusing their patients on preventive care , rather than of simply training patients .
	manualset3
121537	9	404937	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients should have an awareness of their disease , and as health care providers , PD nurses have the role of focusing their patients on preventive care , rather than of simply training patients .
	manualset3
121538	1	404938	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients typically access antiretroviral treatment with advanced symptomatic disease , and mortality is strongly associated with baseline CD4 cell count less than 50 cells/mul and WHO stage 4 disease ( AIDS ) .
	manualset3
121539	2	404938	5	NULL	NULL	0	NULL	antiretroviral treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients typically access antiretroviral treatment with advanced symptomatic disease , and mortality is strongly associated with baseline CD4 cell count less than 50 cells/mul and WHO stage 4 disease ( AIDS ) .
	manualset3
121540	3	404938	5	NULL	NULL	0	NULL	advanced symptomatic disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients typically access antiretroviral treatment with advanced symptomatic disease , and mortality is strongly associated with baseline CD4 cell count less than 50 cells/mul and WHO stage 4 disease ( AIDS ) .
	manualset3
121541	4	404938	5	NULL	NULL	0	NULL	mortality 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients typically access antiretroviral treatment with advanced symptomatic disease , and mortality is strongly associated with baseline CD4 cell count less than 50 cells/mul and WHO stage 4 disease ( AIDS ) .
	manualset3
121542	5	404938	5	NULL	NULL	0	NULL	baseline CD4 cell count	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients typically access antiretroviral treatment with advanced symptomatic disease , and mortality is strongly associated with baseline CD4 cell count less than 50 cells/mul and WHO stage 4 disease ( AIDS ) .
	manualset3
121543	6	404938	5	NULL	NULL	0	NULL	 50 cells/mul	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients typically access antiretroviral treatment with advanced symptomatic disease , and mortality is strongly associated with baseline CD4 cell count less than 50 cells/mul and WHO stage 4 disease ( AIDS ) .
	manualset3
121544	7	404938	5	NULL	NULL	0	NULL	WHO stage 4 disease ( AIDS )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients typically access antiretroviral treatment with advanced symptomatic disease , and mortality is strongly associated with baseline CD4 cell count less than 50 cells/mul and WHO stage 4 disease ( AIDS ) .
	manualset3
121545	1	404939	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing microvascular decompression as a primary procedure were cured ( total pain relief without further therapy ) at a rate of 91 % , versus 43 % in patients treated with destructive procedures ( rhizotomies ) prior to microvascular decompression ( p less than 0.005 ) .
	manualset3
121546	2	404939	5	NULL	NULL	0	NULL	microvascular decompression	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing microvascular decompression as a primary procedure were cured ( total pain relief without further therapy ) at a rate of 91 % , versus 43 % in patients treated with destructive procedures ( rhizotomies ) prior to microvascular decompression ( p less than 0.005 ) .
	manualset3
121547	3	404939	5	NULL	NULL	0	NULL	primary procedure 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing microvascular decompression as a primary procedure were cured ( total pain relief without further therapy ) at a rate of 91 % , versus 43 % in patients treated with destructive procedures ( rhizotomies ) prior to microvascular decompression ( p less than 0.005 ) .
	manualset3
121548	4	404939	5	NULL	NULL	0	NULL	total pain relief	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing microvascular decompression as a primary procedure were cured ( total pain relief without further therapy ) at a rate of 91 % , versus 43 % in patients treated with destructive procedures ( rhizotomies ) prior to microvascular decompression ( p less than 0.005 ) .
	manualset3
121549	5	404939	5	NULL	NULL	0	NULL	therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing microvascular decompression as a primary procedure were cured ( total pain relief without further therapy ) at a rate of 91 % , versus 43 % in patients treated with destructive procedures ( rhizotomies ) prior to microvascular decompression ( p less than 0.005 ) .
	manualset3
121550	6	404939	5	NULL	NULL	0	NULL	rate 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing microvascular decompression as a primary procedure were cured ( total pain relief without further therapy ) at a rate of 91 % , versus 43 % in patients treated with destructive procedures ( rhizotomies ) prior to microvascular decompression ( p less than 0.005 ) .
	manualset3
121551	7	404939	5	NULL	NULL	0	NULL	91 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing microvascular decompression as a primary procedure were cured ( total pain relief without further therapy ) at a rate of 91 % , versus 43 % in patients treated with destructive procedures ( rhizotomies ) prior to microvascular decompression ( p less than 0.005 ) .
	manualset3
121552	8	404939	5	NULL	NULL	NULL	NULL	43 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patients undergoing microvascular decompression as a primary procedure were cured ( total pain relief without further therapy ) at a rate of 91 % , versus 43 % in patients treated with destructive procedures ( rhizotomies ) prior to microvascular decompression ( p less than 0.005 ) .
	manualset3
121553	9	404939	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing microvascular decompression as a primary procedure were cured ( total pain relief without further therapy ) at a rate of 91 % , versus 43 % in patients treated with destructive procedures ( rhizotomies ) prior to microvascular decompression ( p less than 0.005 ) .
	manualset3
121554	10	404939	5	NULL	NULL	0	NULL	destructive procedures ( rhizotomies ) 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing microvascular decompression as a primary procedure were cured ( total pain relief without further therapy ) at a rate of 91 % , versus 43 % in patients treated with destructive procedures ( rhizotomies ) prior to microvascular decompression ( p less than 0.005 ) .
	manualset3
121555	11	404939	5	NULL	NULL	0	NULL	microvascular decompression 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing microvascular decompression as a primary procedure were cured ( total pain relief without further therapy ) at a rate of 91 % , versus 43 % in patients treated with destructive procedures ( rhizotomies ) prior to microvascular decompression ( p less than 0.005 ) .
	manualset3
121556	12	404939	5	NULL	NULL	0	NULL	p less than 0.005	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing microvascular decompression as a primary procedure were cured ( total pain relief without further therapy ) at a rate of 91 % , versus 43 % in patients treated with destructive procedures ( rhizotomies ) prior to microvascular decompression ( p less than 0.005 ) .
	manualset3
121557	1	404940	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing unilateral mandibular 3rd molar extraction surgery were allocated to 3 groups , A , B and C. After oral premedication of meloxicam 10 mg in group A , ampiroxicam 27 mg in group B and placebo in group C , surgery was completed within 30 min under local anaesthesia using 2 % lidocaine .
	manualset3
121558	2	404940	5	NULL	NULL	0	NULL	unilateral mandibular 3rd molar extraction surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing unilateral mandibular 3rd molar extraction surgery were allocated to 3 groups , A , B and C. After oral premedication of meloxicam 10 mg in group A , ampiroxicam 27 mg in group B and placebo in group C , surgery was completed within 30 min under local anaesthesia using 2 % lidocaine .
	manualset3
121559	3	404940	5	NULL	NULL	0	NULL	3 groups , A , B and C	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing unilateral mandibular 3rd molar extraction surgery were allocated to 3 groups , A , B and C. After oral premedication of meloxicam 10 mg in group A , ampiroxicam 27 mg in group B and placebo in group C , surgery was completed within 30 min under local anaesthesia using 2 % lidocaine .
	manualset3
121560	4	404940	5	NULL	NULL	0	NULL	oral premedication	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing unilateral mandibular 3rd molar extraction surgery were allocated to 3 groups , A , B and C. After oral premedication of meloxicam 10 mg in group A , ampiroxicam 27 mg in group B and placebo in group C , surgery was completed within 30 min under local anaesthesia using 2 % lidocaine .
	manualset3
121561	5	404940	5	NULL	NULL	0	NULL	meloxicam	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing unilateral mandibular 3rd molar extraction surgery were allocated to 3 groups , A , B and C. After oral premedication of meloxicam 10 mg in group A , ampiroxicam 27 mg in group B and placebo in group C , surgery was completed within 30 min under local anaesthesia using 2 % lidocaine .
	manualset3
121562	6	404940	5	NULL	NULL	0	NULL	10 mg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing unilateral mandibular 3rd molar extraction surgery were allocated to 3 groups , A , B and C. After oral premedication of meloxicam 10 mg in group A , ampiroxicam 27 mg in group B and placebo in group C , surgery was completed within 30 min under local anaesthesia using 2 % lidocaine .
	manualset3
121563	7	404940	5	NULL	NULL	0	NULL	group A	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing unilateral mandibular 3rd molar extraction surgery were allocated to 3 groups , A , B and C. After oral premedication of meloxicam 10 mg in group A , ampiroxicam 27 mg in group B and placebo in group C , surgery was completed within 30 min under local anaesthesia using 2 % lidocaine .
	manualset3
121564	8	404940	5	NULL	NULL	0	NULL	ampiroxicam 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing unilateral mandibular 3rd molar extraction surgery were allocated to 3 groups , A , B and C. After oral premedication of meloxicam 10 mg in group A , ampiroxicam 27 mg in group B and placebo in group C , surgery was completed within 30 min under local anaesthesia using 2 % lidocaine .
	manualset3
121565	9	404940	5	NULL	NULL	0	NULL	27 mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing unilateral mandibular 3rd molar extraction surgery were allocated to 3 groups , A , B and C. After oral premedication of meloxicam 10 mg in group A , ampiroxicam 27 mg in group B and placebo in group C , surgery was completed within 30 min under local anaesthesia using 2 % lidocaine .
	manualset3
121566	10	404940	5	NULL	NULL	0	NULL	group B	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing unilateral mandibular 3rd molar extraction surgery were allocated to 3 groups , A , B and C. After oral premedication of meloxicam 10 mg in group A , ampiroxicam 27 mg in group B and placebo in group C , surgery was completed within 30 min under local anaesthesia using 2 % lidocaine .
	manualset3
121567	11	404940	5	NULL	NULL	0	NULL	placebo 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing unilateral mandibular 3rd molar extraction surgery were allocated to 3 groups , A , B and C. After oral premedication of meloxicam 10 mg in group A , ampiroxicam 27 mg in group B and placebo in group C , surgery was completed within 30 min under local anaesthesia using 2 % lidocaine .
	manualset3
121568	12	404940	5	NULL	NULL	0	NULL	group C	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing unilateral mandibular 3rd molar extraction surgery were allocated to 3 groups , A , B and C. After oral premedication of meloxicam 10 mg in group A , ampiroxicam 27 mg in group B and placebo in group C , surgery was completed within 30 min under local anaesthesia using 2 % lidocaine .
	manualset3
121569	13	404940	5	NULL	NULL	0	NULL	surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing unilateral mandibular 3rd molar extraction surgery were allocated to 3 groups , A , B and C. After oral premedication of meloxicam 10 mg in group A , ampiroxicam 27 mg in group B and placebo in group C , surgery was completed within 30 min under local anaesthesia using 2 % lidocaine .
	manualset3
121570	14	404940	5	NULL	NULL	0	NULL	 30 min	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing unilateral mandibular 3rd molar extraction surgery were allocated to 3 groups , A , B and C. After oral premedication of meloxicam 10 mg in group A , ampiroxicam 27 mg in group B and placebo in group C , surgery was completed within 30 min under local anaesthesia using 2 % lidocaine .
	manualset3
121571	15	404940	5	NULL	NULL	0	NULL	local anaesthesia	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing unilateral mandibular 3rd molar extraction surgery were allocated to 3 groups , A , B and C. After oral premedication of meloxicam 10 mg in group A , ampiroxicam 27 mg in group B and placebo in group C , surgery was completed within 30 min under local anaesthesia using 2 % lidocaine .
	manualset3
121572	16	404940	5	NULL	NULL	0	NULL	2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing unilateral mandibular 3rd molar extraction surgery were allocated to 3 groups , A , B and C. After oral premedication of meloxicam 10 mg in group A , ampiroxicam 27 mg in group B and placebo in group C , surgery was completed within 30 min under local anaesthesia using 2 % lidocaine .
	manualset3
121573	17	404940	5	NULL	NULL	0	NULL	lidocaine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing unilateral mandibular 3rd molar extraction surgery were allocated to 3 groups , A , B and C. After oral premedication of meloxicam 10 mg in group A , ampiroxicam 27 mg in group B and placebo in group C , surgery was completed within 30 min under local anaesthesia using 2 % lidocaine .
	manualset3
121574	1	404941	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients usually have lowered C4 levels , and diagnosis relies on determination of antigenic and/or functional C1 inhibitor level .
	manualset3
121575	2	404941	5	NULL	NULL	0	NULL	C4 levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients usually have lowered C4 levels , and diagnosis relies on determination of antigenic and/or functional C1 inhibitor level .
	manualset3
121576	3	404941	5	NULL	NULL	NULL	NULL	diagnosis 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patients usually have lowered C4 levels , and diagnosis relies on determination of antigenic and/or functional C1 inhibitor level .
	manualset3
121577	4	404941	5	NULL	NULL	0	NULL	determination 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients usually have lowered C4 levels , and diagnosis relies on determination of antigenic and/or functional C1 inhibitor level .
	manualset3
121578	5	404941	5	NULL	NULL	0	NULL	antigenic and/or functional C1 inhibitor level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients usually have lowered C4 levels , and diagnosis relies on determination of antigenic and/or functional C1 inhibitor level .
	manualset3
121579	1	404942	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients were classified into four groups : primary bacteremia ( PB ) , enteritis-associated bacteremia ( secondary bacteremia ) ( SB ) , digestive focal infection ( DI ) and non-digestive focal infection ( NDI ) .
	manualset3
121580	2	404942	5	NULL	NULL	0	NULL	four groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients were classified into four groups : primary bacteremia ( PB ) , enteritis-associated bacteremia ( secondary bacteremia ) ( SB ) , digestive focal infection ( DI ) and non-digestive focal infection ( NDI ) .
	manualset3
121581	3	404942	5	NULL	NULL	0	NULL	primary bacteremia ( PB )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients were classified into four groups : primary bacteremia ( PB ) , enteritis-associated bacteremia ( secondary bacteremia ) ( SB ) , digestive focal infection ( DI ) and non-digestive focal infection ( NDI ) .
	manualset3
121582	4	404942	5	NULL	NULL	0	NULL	enteritis-associated bacteremia ( secondary bacteremia ) ( SB )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients were classified into four groups : primary bacteremia ( PB ) , enteritis-associated bacteremia ( secondary bacteremia ) ( SB ) , digestive focal infection ( DI ) and non-digestive focal infection ( NDI ) .
	manualset3
121583	5	404942	5	NULL	NULL	0	NULL	digestive focal infection ( DI ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients were classified into four groups : primary bacteremia ( PB ) , enteritis-associated bacteremia ( secondary bacteremia ) ( SB ) , digestive focal infection ( DI ) and non-digestive focal infection ( NDI ) .
	manualset3
121584	6	404942	5	NULL	NULL	0	NULL	non-digestive focal infection ( NDI )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients were classified into four groups : primary bacteremia ( PB ) , enteritis-associated bacteremia ( secondary bacteremia ) ( SB ) , digestive focal infection ( DI ) and non-digestive focal infection ( NDI ) .
	manualset3
121585	1	404943	5	NULL	NULL	NULL	NULL	genetic reform	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A genetic reform of the civil law computations of the degrees of relationship in families .
	manualset3
121586	2	404943	5	NULL	NULL	0	NULL	civil law computations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A genetic reform of the civil law computations of the degrees of relationship in families .
	manualset3
121587	3	404943	5	NULL	NULL	0	NULL	degrees 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A genetic reform of the civil law computations of the degrees of relationship in families .
	manualset3
121588	4	404943	5	NULL	NULL	0	NULL	relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A genetic reform of the civil law computations of the degrees of relationship in families .
	manualset3
121589	5	404943	5	NULL	NULL	0	NULL	families 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A genetic reform of the civil law computations of the degrees of relationship in families .
	manualset3
121590	1	404944	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients were dialyzed for approximately 4 hr between 07 : 00 and 13 : 00 hr ( S1 ) , between 13 : 00 and 20 : 00 hr ( S2 ) , or between 18 : 30 and 22 : 30 hr ( S3 ) .
	manualset3
121591	2	404944	5	NULL	NULL	0	NULL	4 hr	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients were dialyzed for approximately 4 hr between 07 : 00 and 13 : 00 hr ( S1 ) , between 13 : 00 and 20 : 00 hr ( S2 ) , or between 18 : 30 and 22 : 30 hr ( S3 ) .
	manualset3
121592	3	404944	5	NULL	NULL	0	NULL	between 07 : 00 and 13 : 00 hr ( S1 )	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients were dialyzed for approximately 4 hr between 07 : 00 and 13 : 00 hr ( S1 ) , between 13 : 00 and 20 : 00 hr ( S2 ) , or between 18 : 30 and 22 : 30 hr ( S3 ) .
	manualset3
121593	4	404944	5	NULL	NULL	0	NULL	between 13 : 00 and 20 : 00 hr ( S2 )	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients were dialyzed for approximately 4 hr between 07 : 00 and 13 : 00 hr ( S1 ) , between 13 : 00 and 20 : 00 hr ( S2 ) , or between 18 : 30 and 22 : 30 hr ( S3 ) .
	manualset3
121594	5	404944	5	NULL	NULL	0	NULL	between 18 : 30 and 22 : 30 hr ( S3 )	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients were dialyzed for approximately 4 hr between 07 : 00 and 13 : 00 hr ( S1 ) , between 13 : 00 and 20 : 00 hr ( S2 ) , or between 18 : 30 and 22 : 30 hr ( S3 ) .
	manualset3
121595	1	404945	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients were divided into three groups based on the dose of vecuronium given .
	manualset3
121596	2	404945	5	NULL	NULL	NULL	NULL	three groups	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patients were divided into three groups based on the dose of vecuronium given .
	manualset3
121597	3	404945	5	NULL	NULL	0	NULL	dose 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients were divided into three groups based on the dose of vecuronium given .
	manualset3
121598	4	404945	5	NULL	NULL	0	NULL	vecuronium 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients were divided into three groups based on the dose of vecuronium given .
	manualset3
121599	1	404946	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients were grafted with a median number of 4.1 x 10 ( 6 ) kg ( 1.6-6 .4 ) CD34 + cells and 0.42 x 10 ( 6 ) / kg ( 0.29-2 .2 ) CD3 + cells .
	manualset3
121600	2	404946	5	NULL	NULL	0	NULL	median number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients were grafted with a median number of 4.1 x 10 ( 6 ) kg ( 1.6-6 .4 ) CD34 + cells and 0.42 x 10 ( 6 ) / kg ( 0.29-2 .2 ) CD3 + cells .
	manualset3
121601	3	404946	5	NULL	NULL	0	NULL	 4.1 x 10 ( 6 ) kg ( 1.6-6 .4 ) CD34 + cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients were grafted with a median number of 4.1 x 10 ( 6 ) kg ( 1.6-6 .4 ) CD34 + cells and 0.42 x 10 ( 6 ) / kg ( 0.29-2 .2 ) CD3 + cells .
	manualset3
121602	4	404946	5	NULL	NULL	0	NULL	0.42 x 10 ( 6 ) / kg ( 0.29-2 .2 ) CD3 + cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients were grafted with a median number of 4.1 x 10 ( 6 ) kg ( 1.6-6 .4 ) CD34 + cells and 0.42 x 10 ( 6 ) / kg ( 0.29-2 .2 ) CD3 + cells .
	manualset3
121603	1	404947	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients who suffer superficial recurrences of breast cancer , be it in their chest wall following mastectomy , or in their breast after breast conservation , typically have poor clinical outcomes .
	manualset3
121604	2	404947	5	NULL	NULL	0	NULL	superficial recurrences 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients who suffer superficial recurrences of breast cancer , be it in their chest wall following mastectomy , or in their breast after breast conservation , typically have poor clinical outcomes .
	manualset3
121605	3	404947	5	NULL	NULL	0	NULL	breast cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients who suffer superficial recurrences of breast cancer , be it in their chest wall following mastectomy , or in their breast after breast conservation , typically have poor clinical outcomes .
	manualset3
121606	4	404947	5	NULL	NULL	0	NULL	chest wall	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients who suffer superficial recurrences of breast cancer , be it in their chest wall following mastectomy , or in their breast after breast conservation , typically have poor clinical outcomes .
	manualset3
121607	5	404947	5	NULL	NULL	0	NULL	mastectomy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients who suffer superficial recurrences of breast cancer , be it in their chest wall following mastectomy , or in their breast after breast conservation , typically have poor clinical outcomes .
	manualset3
121608	6	404947	5	NULL	NULL	0	NULL	breast 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients who suffer superficial recurrences of breast cancer , be it in their chest wall following mastectomy , or in their breast after breast conservation , typically have poor clinical outcomes .
	manualset3
121609	7	404947	5	NULL	NULL	0	NULL	breast conservation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients who suffer superficial recurrences of breast cancer , be it in their chest wall following mastectomy , or in their breast after breast conservation , typically have poor clinical outcomes .
	manualset3
121610	8	404947	5	NULL	NULL	0	NULL	poor clinical outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients who suffer superficial recurrences of breast cancer , be it in their chest wall following mastectomy , or in their breast after breast conservation , typically have poor clinical outcomes .
	manualset3
121611	1	404948	5	NULL	NULL	0	NULL	COAGULATION DISORDERS 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( COAGULATION DISORDERS CAUSED BY RETENTION OF A DEAD FETUS AND THEIR MANAGEMENT ) .
	manualset3
121612	2	404948	5	NULL	NULL	0	NULL	RETENTION 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( COAGULATION DISORDERS CAUSED BY RETENTION OF A DEAD FETUS AND THEIR MANAGEMENT ) .
	manualset3
121613	3	404948	5	NULL	NULL	NULL	NULL	DEAD FETUS 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( COAGULATION DISORDERS CAUSED BY RETENTION OF A DEAD FETUS AND THEIR MANAGEMENT ) .
	manualset3
121614	4	404948	5	NULL	NULL	0	NULL	MANAGEMENT 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( COAGULATION DISORDERS CAUSED BY RETENTION OF A DEAD FETUS AND THEIR MANAGEMENT ) .
	manualset3
121615	1	404949	5	NULL	NULL	0	NULL	genetic screen	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A genetic screen for modifiers of Drosophila caspase Dcp-1 reveals caspase involvement in autophagy and novel caspase-related genes .
	manualset3
121616	2	404949	5	NULL	NULL	NULL	NULL	modifiers of Drosophila caspase Dcp-1	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A genetic screen for modifiers of Drosophila caspase Dcp-1 reveals caspase involvement in autophagy and novel caspase-related genes .
	manualset3
121617	3	404949	5	NULL	NULL	0	NULL	caspase 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A genetic screen for modifiers of Drosophila caspase Dcp-1 reveals caspase involvement in autophagy and novel caspase-related genes .
	manualset3
121618	4	404949	5	NULL	NULL	0	NULL	autophagy 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A genetic screen for modifiers of Drosophila caspase Dcp-1 reveals caspase involvement in autophagy and novel caspase-related genes .
	manualset3
121619	5	404949	5	NULL	NULL	0	NULL	novel caspase-related genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A genetic screen for modifiers of Drosophila caspase Dcp-1 reveals caspase involvement in autophagy and novel caspase-related genes .
	manualset3
121620	1	404950	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients whose outflow resistance is increased in the ventricular infusion test but with a physiological lumbar infusion test are suspected for a functional aqueduct stenosis and should be treated by means of an endoscopic assisted ventriculostomy .
	manualset3
121621	2	404950	5	NULL	NULL	0	NULL	outflow resistance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients whose outflow resistance is increased in the ventricular infusion test but with a physiological lumbar infusion test are suspected for a functional aqueduct stenosis and should be treated by means of an endoscopic assisted ventriculostomy .
	manualset3
121622	3	404950	5	NULL	NULL	0	NULL	ventricular infusion test	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients whose outflow resistance is increased in the ventricular infusion test but with a physiological lumbar infusion test are suspected for a functional aqueduct stenosis and should be treated by means of an endoscopic assisted ventriculostomy .
	manualset3
121623	4	404950	5	NULL	NULL	0	NULL	physiological lumbar infusion test 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients whose outflow resistance is increased in the ventricular infusion test but with a physiological lumbar infusion test are suspected for a functional aqueduct stenosis and should be treated by means of an endoscopic assisted ventriculostomy .
	manualset3
121624	5	404950	5	NULL	NULL	0	NULL	functional aqueduct stenosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients whose outflow resistance is increased in the ventricular infusion test but with a physiological lumbar infusion test are suspected for a functional aqueduct stenosis and should be treated by means of an endoscopic assisted ventriculostomy .
	manualset3
121625	6	404950	5	NULL	NULL	0	NULL	endoscopic assisted ventriculostomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients whose outflow resistance is increased in the ventricular infusion test but with a physiological lumbar infusion test are suspected for a functional aqueduct stenosis and should be treated by means of an endoscopic assisted ventriculostomy .
	manualset3
121626	1	404951	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with ITPA 94C ) A homozygous allele are at high risk to develop AZA-related gastrointestinal toxicity and flu-like symptoms ( P & lt ; 0.01 ) .
	manualset3
121627	2	404951	5	NULL	NULL	0	NULL	ITPA 94C ) A homozygous allele	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with ITPA 94C ) A homozygous allele are at high risk to develop AZA-related gastrointestinal toxicity and flu-like symptoms ( P & lt ; 0.01 ) .
	manualset3
121628	3	404951	5	NULL	NULL	0	NULL	high risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with ITPA 94C ) A homozygous allele are at high risk to develop AZA-related gastrointestinal toxicity and flu-like symptoms ( P & lt ; 0.01 ) .
	manualset3
121629	4	404951	5	NULL	NULL	0	NULL	AZA-related gastrointestinal toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with ITPA 94C ) A homozygous allele are at high risk to develop AZA-related gastrointestinal toxicity and flu-like symptoms ( P & lt ; 0.01 ) .
	manualset3
121630	5	404951	5	NULL	NULL	0	NULL	flu-like symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with ITPA 94C ) A homozygous allele are at high risk to develop AZA-related gastrointestinal toxicity and flu-like symptoms ( P & lt ; 0.01 ) .
	manualset3
121631	6	404951	5	NULL	NULL	0	NULL	 P & lt ; 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with ITPA 94C ) A homozygous allele are at high risk to develop AZA-related gastrointestinal toxicity and flu-like symptoms ( P & lt ; 0.01 ) .
	manualset3
121632	1	404952	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with MetS are more prone to developing cardiovascular events than other patients .
	manualset3
121633	2	404952	5	NULL	NULL	0	NULL	MetS 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with MetS are more prone to developing cardiovascular events than other patients .
	manualset3
121634	3	404952	5	NULL	NULL	0	NULL	cardiovascular events	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with MetS are more prone to developing cardiovascular events than other patients .
	manualset3
121635	4	404952	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with MetS are more prone to developing cardiovascular events than other patients .
	manualset3
121636	1	404953	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with Parkinson 's disease demonstrated an impairment in appetitive motivational arousal consistent with the progression of dopaminergic degeneration across the course of the disease .
	manualset3
121637	2	404953	5	NULL	NULL	0	NULL	Parkinson 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with Parkinson 's disease demonstrated an impairment in appetitive motivational arousal consistent with the progression of dopaminergic degeneration across the course of the disease .
	manualset3
121638	3	404953	5	NULL	NULL	0	NULL	impairment in appetitive motivational arousal 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with Parkinson 's disease demonstrated an impairment in appetitive motivational arousal consistent with the progression of dopaminergic degeneration across the course of the disease .
	manualset3
121639	4	404953	5	NULL	NULL	0	NULL	progression 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with Parkinson 's disease demonstrated an impairment in appetitive motivational arousal consistent with the progression of dopaminergic degeneration across the course of the disease .
	manualset3
121640	5	404953	5	NULL	NULL	0	NULL	dopaminergic degeneration 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with Parkinson 's disease demonstrated an impairment in appetitive motivational arousal consistent with the progression of dopaminergic degeneration across the course of the disease .
	manualset3
121641	6	404953	5	NULL	NULL	0	NULL	course 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with Parkinson 's disease demonstrated an impairment in appetitive motivational arousal consistent with the progression of dopaminergic degeneration across the course of the disease .
	manualset3
121642	7	404953	5	NULL	NULL	0	NULL	disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with Parkinson 's disease demonstrated an impairment in appetitive motivational arousal consistent with the progression of dopaminergic degeneration across the course of the disease .
	manualset3
121643	1	404954	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with RA appear to have less capacity for excreting paracetamol as non-toxic conjugates and may be more susceptible to paracetamol toxicity , especially on chronic dosage .
	manualset3
121644	2	404954	5	NULL	NULL	0	NULL	RA 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with RA appear to have less capacity for excreting paracetamol as non-toxic conjugates and may be more susceptible to paracetamol toxicity , especially on chronic dosage .
	manualset3
121645	3	404954	5	NULL	NULL	0	NULL	less capacity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with RA appear to have less capacity for excreting paracetamol as non-toxic conjugates and may be more susceptible to paracetamol toxicity , especially on chronic dosage .
	manualset3
121646	4	404954	5	NULL	NULL	0	NULL	paracetamol 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with RA appear to have less capacity for excreting paracetamol as non-toxic conjugates and may be more susceptible to paracetamol toxicity , especially on chronic dosage .
	manualset3
121647	5	404954	5	NULL	NULL	0	NULL	non-toxic conjugates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with RA appear to have less capacity for excreting paracetamol as non-toxic conjugates and may be more susceptible to paracetamol toxicity , especially on chronic dosage .
	manualset3
121648	6	404954	5	NULL	NULL	0	NULL	paracetamol toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with RA appear to have less capacity for excreting paracetamol as non-toxic conjugates and may be more susceptible to paracetamol toxicity , especially on chronic dosage .
	manualset3
121649	7	404954	5	NULL	NULL	0	NULL	chronic dosage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with RA appear to have less capacity for excreting paracetamol as non-toxic conjugates and may be more susceptible to paracetamol toxicity , especially on chronic dosage .
	manualset3
121650	1	404955	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with Turner syndrome have many somatic characteristics , including short stature .
	manualset3
121651	2	404955	5	NULL	NULL	0	NULL	Turner syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with Turner syndrome have many somatic characteristics , including short stature .
	manualset3
121652	3	404955	5	NULL	NULL	0	NULL	somatic characteristics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with Turner syndrome have many somatic characteristics , including short stature .
	manualset3
121653	4	404955	5	NULL	NULL	0	NULL	short stature 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with Turner syndrome have many somatic characteristics , including short stature .
	manualset3
121654	1	404956	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with a history of herpetic CNS disease should be warned to immediately report any visual symptoms .
	manualset3
121655	2	404956	5	NULL	NULL	0	NULL	history 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with a history of herpetic CNS disease should be warned to immediately report any visual symptoms .
	manualset3
121656	3	404956	5	NULL	NULL	0	NULL	herpetic CNS disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with a history of herpetic CNS disease should be warned to immediately report any visual symptoms .
	manualset3
121658	4	404956	5	NULL	NULL	NULL	NULL	visual symptoms	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patients with a history of herpetic CNS disease should be warned to immediately report any visual symptoms .
	manualset3
121659	1	404957	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with a narrow face have often a defect in expansion of the maxillary-malar complex .
	manualset3
121660	2	404957	5	NULL	NULL	0	NULL	narrow face	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with a narrow face have often a defect in expansion of the maxillary-malar complex .
	manualset3
121661	3	404957	5	NULL	NULL	0	NULL	defect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with a narrow face have often a defect in expansion of the maxillary-malar complex .
	manualset3
121662	4	404957	5	NULL	NULL	0	NULL	expansion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with a narrow face have often a defect in expansion of the maxillary-malar complex .
	manualset3
121663	5	404957	5	NULL	NULL	0	NULL	maxillary-malar complex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with a narrow face have often a defect in expansion of the maxillary-malar complex .
	manualset3
121664	1	404958	5	NULL	NULL	0	NULL	genetic variation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A genetic variation between the strains was observed after phenobarbital ( PB ) treatment in the content of cytochrome P-450 and in the various enzyme activities , varying from non-responsiveness to a 4 - to 5-fold increase .
	manualset3
121665	2	404958	5	NULL	NULL	0	NULL	strains 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A genetic variation between the strains was observed after phenobarbital ( PB ) treatment in the content of cytochrome P-450 and in the various enzyme activities , varying from non-responsiveness to a 4 - to 5-fold increase .
	manualset3
121666	3	404958	5	NULL	NULL	0	NULL	phenobarbital ( PB ) treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A genetic variation between the strains was observed after phenobarbital ( PB ) treatment in the content of cytochrome P-450 and in the various enzyme activities , varying from non-responsiveness to a 4 - to 5-fold increase .
	manualset3
121667	4	404958	5	NULL	NULL	0	NULL	content 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A genetic variation between the strains was observed after phenobarbital ( PB ) treatment in the content of cytochrome P-450 and in the various enzyme activities , varying from non-responsiveness to a 4 - to 5-fold increase .
	manualset3
121668	5	404958	5	NULL	NULL	0	NULL	cytochrome P-450 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A genetic variation between the strains was observed after phenobarbital ( PB ) treatment in the content of cytochrome P-450 and in the various enzyme activities , varying from non-responsiveness to a 4 - to 5-fold increase .
	manualset3
121669	6	404958	5	NULL	NULL	0	NULL	various enzyme activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A genetic variation between the strains was observed after phenobarbital ( PB ) treatment in the content of cytochrome P-450 and in the various enzyme activities , varying from non-responsiveness to a 4 - to 5-fold increase .
	manualset3
121671	8	404958	5	NULL	NULL	NULL	NULL	4 - to 5-fold increase	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A genetic variation between the strains was observed after phenobarbital ( PB ) treatment in the content of cytochrome P-450 and in the various enzyme activities , varying from non-responsiveness to a 4 - to 5-fold increase .
	manualset3
128807	7	404958	5	NULL	NULL	0	NULL	non-responsiveness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A genetic variation between the strains was observed after phenobarbital ( PB ) treatment in the content of cytochrome P-450 and in the various enzyme activities , varying from non-responsiveness to a 4 - to 5-fold increase .
	manualset3
121672	1	404959	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with a posterior disruption of the pelvis had a higher mortality , a higher `` injury severity score , '' and required greater resuscitation efforts .
	manualset3
121673	2	404959	5	NULL	NULL	0	NULL	posterior disruption 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with a posterior disruption of the pelvis had a higher mortality , a higher `` injury severity score , '' and required greater resuscitation efforts .
	manualset3
121674	3	404959	5	NULL	NULL	NULL	NULL	pelvis 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patients with a posterior disruption of the pelvis had a higher mortality , a higher `` injury severity score , '' and required greater resuscitation efforts .
	manualset3
121675	4	404959	5	NULL	NULL	NULL	NULL	higher mortality 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patients with a posterior disruption of the pelvis had a higher mortality , a higher `` injury severity score , '' and required greater resuscitation efforts .
	manualset3
121677	5	404959	5	NULL	NULL	0	NULL	 injury severity score	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with a posterior disruption of the pelvis had a higher mortality , a higher `` injury severity score , '' and required greater resuscitation efforts .
	manualset3
121678	6	404959	5	NULL	NULL	0	NULL	resuscitation efforts	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with a posterior disruption of the pelvis had a higher mortality , a higher `` injury severity score , '' and required greater resuscitation efforts .
	manualset3
121679	1	404960	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with above-average pretreatment distrust and alienation scores more frequently failed to return the follow-up form than patients with below-average scores .
	manualset3
121680	2	404960	5	NULL	NULL	NULL	NULL	above-average pretreatment distrust and alienation scores 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patients with above-average pretreatment distrust and alienation scores more frequently failed to return the follow-up form than patients with below-average scores .
	manualset3
121683	3	404960	5	NULL	NULL	0	NULL	follow-up form 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with above-average pretreatment distrust and alienation scores more frequently failed to return the follow-up form than patients with below-average scores .
	manualset3
121684	4	404960	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with above-average pretreatment distrust and alienation scores more frequently failed to return the follow-up form than patients with below-average scores .
	manualset3
121685	5	404960	5	NULL	NULL	0	NULL	below-average scores	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with above-average pretreatment distrust and alienation scores more frequently failed to return the follow-up form than patients with below-average scores .
	manualset3
121755	1	404961	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with aggressive bladder cancer had a similar distribution but significantly lower mean value ( p & lt ; 0.005 ) .
	manualset3
121756	2	404961	5	NULL	NULL	0	NULL	aggressive bladder cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with aggressive bladder cancer had a similar distribution but significantly lower mean value ( p & lt ; 0.005 ) .
	manualset3
121757	3	404961	5	NULL	NULL	0	NULL	distribution 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with aggressive bladder cancer had a similar distribution but significantly lower mean value ( p & lt ; 0.005 ) .
	manualset3
121758	4	404961	5	NULL	NULL	0	NULL	lower mean value 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with aggressive bladder cancer had a similar distribution but significantly lower mean value ( p & lt ; 0.005 ) .
	manualset3
121759	5	404961	5	NULL	NULL	0	NULL	p & lt ; 0.005	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with aggressive bladder cancer had a similar distribution but significantly lower mean value ( p & lt ; 0.005 ) .
	manualset3
121760	1	404962	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with an APOE 4 allele had significantly less motor recovery during rehabilitation than did patients without an APOE 4 allele ( mean 3.7 vs. 6.1 ; P = 0.04 ) and a longer rehabilitation length of stay ( LOS ) ( mean 117.4 vs. 94.5 ; P = 0.02 ) , but better sensory-pinprick recovery ( mean 6.1 vs. 4.0 ; P = 0.03 ) .
	manualset3
121761	2	404962	5	NULL	NULL	0	NULL	APOE 4 allele	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with an APOE 4 allele had significantly less motor recovery during rehabilitation than did patients without an APOE 4 allele ( mean 3.7 vs. 6.1 ; P = 0.04 ) and a longer rehabilitation length of stay ( LOS ) ( mean 117.4 vs. 94.5 ; P = 0.02 ) , but better sensory-pinprick recovery ( mean 6.1 vs. 4.0 ; P = 0.03 ) .
	manualset3
121762	3	404962	5	NULL	NULL	0	NULL	motor recovery	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with an APOE 4 allele had significantly less motor recovery during rehabilitation than did patients without an APOE 4 allele ( mean 3.7 vs. 6.1 ; P = 0.04 ) and a longer rehabilitation length of stay ( LOS ) ( mean 117.4 vs. 94.5 ; P = 0.02 ) , but better sensory-pinprick recovery ( mean 6.1 vs. 4.0 ; P = 0.03 ) .
	manualset3
121763	4	404962	5	NULL	NULL	0	NULL	rehabilitation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with an APOE 4 allele had significantly less motor recovery during rehabilitation than did patients without an APOE 4 allele ( mean 3.7 vs. 6.1 ; P = 0.04 ) and a longer rehabilitation length of stay ( LOS ) ( mean 117.4 vs. 94.5 ; P = 0.02 ) , but better sensory-pinprick recovery ( mean 6.1 vs. 4.0 ; P = 0.03 ) .
	manualset3
121764	5	404962	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with an APOE 4 allele had significantly less motor recovery during rehabilitation than did patients without an APOE 4 allele ( mean 3.7 vs. 6.1 ; P = 0.04 ) and a longer rehabilitation length of stay ( LOS ) ( mean 117.4 vs. 94.5 ; P = 0.02 ) , but better sensory-pinprick recovery ( mean 6.1 vs. 4.0 ; P = 0.03 ) .
	manualset3
121765	6	404962	5	NULL	NULL	0	NULL	APOE 4 allele	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with an APOE 4 allele had significantly less motor recovery during rehabilitation than did patients without an APOE 4 allele ( mean 3.7 vs. 6.1 ; P = 0.04 ) and a longer rehabilitation length of stay ( LOS ) ( mean 117.4 vs. 94.5 ; P = 0.02 ) , but better sensory-pinprick recovery ( mean 6.1 vs. 4.0 ; P = 0.03 ) .
	manualset3
121766	7	404962	5	NULL	NULL	0	NULL	mean 3.7 vs. 6.1 ; P = 0.04	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with an APOE 4 allele had significantly less motor recovery during rehabilitation than did patients without an APOE 4 allele ( mean 3.7 vs. 6.1 ; P = 0.04 ) and a longer rehabilitation length of stay ( LOS ) ( mean 117.4 vs. 94.5 ; P = 0.02 ) , but better sensory-pinprick recovery ( mean 6.1 vs. 4.0 ; P = 0.03 ) .
	manualset3
121767	8	404962	5	NULL	NULL	NULL	NULL	longer rehabilitation length of stay ( LOS )	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patients with an APOE 4 allele had significantly less motor recovery during rehabilitation than did patients without an APOE 4 allele ( mean 3.7 vs. 6.1 ; P = 0.04 ) and a longer rehabilitation length of stay ( LOS ) ( mean 117.4 vs. 94.5 ; P = 0.02 ) , but better sensory-pinprick recovery ( mean 6.1 vs. 4.0 ; P = 0.03 ) .
	manualset3
121768	9	404962	5	NULL	NULL	0	NULL	mean 117.4 vs. 94.5 ; P = 0.02 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with an APOE 4 allele had significantly less motor recovery during rehabilitation than did patients without an APOE 4 allele ( mean 3.7 vs. 6.1 ; P = 0.04 ) and a longer rehabilitation length of stay ( LOS ) ( mean 117.4 vs. 94.5 ; P = 0.02 ) , but better sensory-pinprick recovery ( mean 6.1 vs. 4.0 ; P = 0.03 ) .
	manualset3
121769	10	404962	5	NULL	NULL	0	NULL	sensory-pinprick recovery	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with an APOE 4 allele had significantly less motor recovery during rehabilitation than did patients without an APOE 4 allele ( mean 3.7 vs. 6.1 ; P = 0.04 ) and a longer rehabilitation length of stay ( LOS ) ( mean 117.4 vs. 94.5 ; P = 0.02 ) , but better sensory-pinprick recovery ( mean 6.1 vs. 4.0 ; P = 0.03 ) .
	manualset3
121770	11	404962	5	NULL	NULL	0	NULL	mean 6.1 vs. 4.0 ; P = 0.03	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with an APOE 4 allele had significantly less motor recovery during rehabilitation than did patients without an APOE 4 allele ( mean 3.7 vs. 6.1 ; P = 0.04 ) and a longer rehabilitation length of stay ( LOS ) ( mean 117.4 vs. 94.5 ; P = 0.02 ) , but better sensory-pinprick recovery ( mean 6.1 vs. 4.0 ; P = 0.03 ) .
	manualset3
121771	1	404963	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with chronic HCV had greater HRQL impairment than healthy controls and those with type II diabetes .
	manualset3
121772	2	404963	5	NULL	NULL	0	NULL	chronic HCV	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with chronic HCV had greater HRQL impairment than healthy controls and those with type II diabetes .
	manualset3
121773	3	404963	5	NULL	NULL	0	NULL	HRQL impairment 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with chronic HCV had greater HRQL impairment than healthy controls and those with type II diabetes .
	manualset3
121774	4	404963	5	NULL	NULL	0	NULL	healthy controls 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with chronic HCV had greater HRQL impairment than healthy controls and those with type II diabetes .
	manualset3
121775	5	404963	5	NULL	NULL	0	NULL	 type II diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with chronic HCV had greater HRQL impairment than healthy controls and those with type II diabetes .
	manualset3
121781	1	404964	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with chronic renal failure , not on hemodialysis , had only mildly depressed neutrophil chemotactic responsiveness ( 42.3 + / -15 ; p less than 0.01 ) .
	manualset3
121783	2	404964	5	NULL	NULL	0	NULL	chronic renal failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with chronic renal failure , not on hemodialysis , had only mildly depressed neutrophil chemotactic responsiveness ( 42.3 + / -15 ; p less than 0.01 ) .
	manualset3
121785	3	404964	5	NULL	NULL	0	NULL	hemodialysis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with chronic renal failure , not on hemodialysis , had only mildly depressed neutrophil chemotactic responsiveness ( 42.3 + / -15 ; p less than 0.01 ) .
	manualset3
121786	4	404964	5	NULL	NULL	0	NULL	mildly depressed neutrophil chemotactic responsiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with chronic renal failure , not on hemodialysis , had only mildly depressed neutrophil chemotactic responsiveness ( 42.3 + / -15 ; p less than 0.01 ) .
	manualset3
121787	5	404964	5	NULL	NULL	0	NULL	42.3 + / -15 ; p less than 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with chronic renal failure , not on hemodialysis , had only mildly depressed neutrophil chemotactic responsiveness ( 42.3 + / -15 ; p less than 0.01 ) .
	manualset3
121788	1	404965	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with evidence of deep venous disease because of reflux or obstruction in the deep veins on Doppler and duplex ultrasonic examination or with an ambulatory venous pressure greater than 45 mm Hg despite the ankle cuff had venography .
	manualset3
121807	2	404965	5	NULL	NULL	0	NULL	evidence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with evidence of deep venous disease because of reflux or obstruction in the deep veins on Doppler and duplex ultrasonic examination or with an ambulatory venous pressure greater than 45 mm Hg despite the ankle cuff had venography .
	manualset3
121808	3	404965	5	NULL	NULL	0	NULL	deep venous disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with evidence of deep venous disease because of reflux or obstruction in the deep veins on Doppler and duplex ultrasonic examination or with an ambulatory venous pressure greater than 45 mm Hg despite the ankle cuff had venography .
	manualset3
121809	4	404965	5	NULL	NULL	0	NULL	reflux 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with evidence of deep venous disease because of reflux or obstruction in the deep veins on Doppler and duplex ultrasonic examination or with an ambulatory venous pressure greater than 45 mm Hg despite the ankle cuff had venography .
	manualset3
121810	5	404965	5	NULL	NULL	0	NULL	obstruction 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with evidence of deep venous disease because of reflux or obstruction in the deep veins on Doppler and duplex ultrasonic examination or with an ambulatory venous pressure greater than 45 mm Hg despite the ankle cuff had venography .
	manualset3
121811	6	404965	5	NULL	NULL	0	NULL	deep veins	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with evidence of deep venous disease because of reflux or obstruction in the deep veins on Doppler and duplex ultrasonic examination or with an ambulatory venous pressure greater than 45 mm Hg despite the ankle cuff had venography .
	manualset3
121812	7	404965	5	NULL	NULL	0	NULL	Doppler and duplex ultrasonic examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with evidence of deep venous disease because of reflux or obstruction in the deep veins on Doppler and duplex ultrasonic examination or with an ambulatory venous pressure greater than 45 mm Hg despite the ankle cuff had venography .
	manualset3
121877	8	404965	5	NULL	NULL	0	NULL	ambulatory venous pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with evidence of deep venous disease because of reflux or obstruction in the deep veins on Doppler and duplex ultrasonic examination or with an ambulatory venous pressure greater than 45 mm Hg despite the ankle cuff had venography .
	manualset3
121878	9	404965	5	NULL	NULL	0	NULL	45 mm Hg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with evidence of deep venous disease because of reflux or obstruction in the deep veins on Doppler and duplex ultrasonic examination or with an ambulatory venous pressure greater than 45 mm Hg despite the ankle cuff had venography .
	manualset3
121879	10	404965	5	NULL	NULL	0	NULL	ankle cuff 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with evidence of deep venous disease because of reflux or obstruction in the deep veins on Doppler and duplex ultrasonic examination or with an ambulatory venous pressure greater than 45 mm Hg despite the ankle cuff had venography .
	manualset3
121880	11	404965	5	NULL	NULL	0	NULL	venography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with evidence of deep venous disease because of reflux or obstruction in the deep veins on Doppler and duplex ultrasonic examination or with an ambulatory venous pressure greater than 45 mm Hg despite the ankle cuff had venography .
	manualset3
121881	1	404966	5	NULL	NULL	0	NULL	genome-wide analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A genome-wide analysis reveals no nuclear dobzhansky-muller pairs of determinants of speciation between S. cerevisiae and S. paradoxus , but suggests more complex incompatibilities .
	manualset3
121883	2	404966	5	NULL	NULL	0	NULL	nuclear dobzhansky-muller pairs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A genome-wide analysis reveals no nuclear dobzhansky-muller pairs of determinants of speciation between S. cerevisiae and S. paradoxus , but suggests more complex incompatibilities .
	manualset3
121913	3	404966	5	NULL	NULL	NULL	NULL	determinants of speciation 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A genome-wide analysis reveals no nuclear dobzhansky-muller pairs of determinants of speciation between S. cerevisiae and S. paradoxus , but suggests more complex incompatibilities .
	manualset3
121917	4	404966	5	NULL	NULL	0	NULL	S. cerevisiae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A genome-wide analysis reveals no nuclear dobzhansky-muller pairs of determinants of speciation between S. cerevisiae and S. paradoxus , but suggests more complex incompatibilities .
	manualset3
121918	5	404966	5	NULL	NULL	0	NULL	 S. paradoxus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A genome-wide analysis reveals no nuclear dobzhansky-muller pairs of determinants of speciation between S. cerevisiae and S. paradoxus , but suggests more complex incompatibilities .
	manualset3
121919	6	404966	5	NULL	NULL	0	NULL	complex incompatibilities 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A genome-wide analysis reveals no nuclear dobzhansky-muller pairs of determinants of speciation between S. cerevisiae and S. paradoxus , but suggests more complex incompatibilities .
	manualset3
121923	1	404967	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with lower nRF values at pre-RT , or a larger increase in nRF from pre-RT to post-RT , had significantly longer PFS .
	manualset3
121924	2	404967	5	NULL	NULL	0	NULL	lower nRF values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with lower nRF values at pre-RT , or a larger increase in nRF from pre-RT to post-RT , had significantly longer PFS .
	manualset3
121925	3	404967	5	NULL	NULL	0	NULL	pre-RT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with lower nRF values at pre-RT , or a larger increase in nRF from pre-RT to post-RT , had significantly longer PFS .
	manualset3
121926	4	404967	5	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with lower nRF values at pre-RT , or a larger increase in nRF from pre-RT to post-RT , had significantly longer PFS .
	manualset3
121927	5	404967	5	NULL	NULL	0	NULL	nRF	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with lower nRF values at pre-RT , or a larger increase in nRF from pre-RT to post-RT , had significantly longer PFS .
	manualset3
121928	6	404967	5	NULL	NULL	0	NULL	pre-RT 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with lower nRF values at pre-RT , or a larger increase in nRF from pre-RT to post-RT , had significantly longer PFS .
	manualset3
121929	7	404967	5	NULL	NULL	0	NULL	post-RT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with lower nRF values at pre-RT , or a larger increase in nRF from pre-RT to post-RT , had significantly longer PFS .
	manualset3
121930	8	404967	5	NULL	NULL	0	NULL	PFS 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with lower nRF values at pre-RT , or a larger increase in nRF from pre-RT to post-RT , had significantly longer PFS .
	manualset3
121931	1	404968	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with major depression showed significantly decreased lymphocyte stimulation induced by PHA , Con A , and PWM as compared to those with minor depression .
	manualset3
121933	2	404968	5	NULL	NULL	0	NULL	major depression	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with major depression showed significantly decreased lymphocyte stimulation induced by PHA , Con A , and PWM as compared to those with minor depression .
	manualset3
121935	3	404968	5	NULL	NULL	0	NULL	lymphocyte stimulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with major depression showed significantly decreased lymphocyte stimulation induced by PHA , Con A , and PWM as compared to those with minor depression .
	manualset3
121940	4	404968	5	NULL	NULL	0	NULL	PHA 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with major depression showed significantly decreased lymphocyte stimulation induced by PHA , Con A , and PWM as compared to those with minor depression .
	manualset3
121941	5	404968	5	NULL	NULL	0	NULL	Con A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with major depression showed significantly decreased lymphocyte stimulation induced by PHA , Con A , and PWM as compared to those with minor depression .
	manualset3
121947	6	404968	5	NULL	NULL	0	NULL	PWM 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with major depression showed significantly decreased lymphocyte stimulation induced by PHA , Con A , and PWM as compared to those with minor depression .
	manualset3
121948	7	404968	5	NULL	NULL	0	NULL	minor depression	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with major depression showed significantly decreased lymphocyte stimulation induced by PHA , Con A , and PWM as compared to those with minor depression .
	manualset3
121952	1	404969	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with obsessive-compulsive disorder may experience severely disabling symptoms and require hospitalization .
	manualset3
121956	2	404969	5	NULL	NULL	0	NULL	obsessive-compulsive disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with obsessive-compulsive disorder may experience severely disabling symptoms and require hospitalization .
	manualset3
121958	3	404969	5	NULL	NULL	NULL	NULL	severely disabling symptoms 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patients with obsessive-compulsive disorder may experience severely disabling symptoms and require hospitalization .
	manualset3
121959	4	404969	5	NULL	NULL	NULL	NULL	hospitalization 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patients with obsessive-compulsive disorder may experience severely disabling symptoms and require hospitalization .
	manualset3
121960	1	404970	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with prefrontal lesions , however , also exhibited working memory deficits on a non-temporal task ( Expt .
	manualset3
121961	2	404970	5	NULL	NULL	0	NULL	prefrontal lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with prefrontal lesions , however , also exhibited working memory deficits on a non-temporal task ( Expt .
	manualset3
121962	3	404970	5	NULL	NULL	0	NULL	working memory deficits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with prefrontal lesions , however , also exhibited working memory deficits on a non-temporal task ( Expt .
	manualset3
121963	4	404970	5	NULL	NULL	0	NULL	non-temporal task	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with prefrontal lesions , however , also exhibited working memory deficits on a non-temporal task ( Expt .
	manualset3
121964	1	404971	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with renal failure caused by acute injury or hepatorenal syndrome have classically not been included as candidates for combined transplantation because of the reversibility of renal dysfunction after liver transplantation .
	manualset3
121965	2	404971	5	NULL	NULL	0	NULL	renal failure 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with renal failure caused by acute injury or hepatorenal syndrome have classically not been included as candidates for combined transplantation because of the reversibility of renal dysfunction after liver transplantation .
	manualset3
121966	3	404971	5	NULL	NULL	0	NULL	acute injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with renal failure caused by acute injury or hepatorenal syndrome have classically not been included as candidates for combined transplantation because of the reversibility of renal dysfunction after liver transplantation .
	manualset3
121967	4	404971	5	NULL	NULL	0	NULL	hepatorenal syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with renal failure caused by acute injury or hepatorenal syndrome have classically not been included as candidates for combined transplantation because of the reversibility of renal dysfunction after liver transplantation .
	manualset3
121968	5	404971	5	NULL	NULL	0	NULL	candidates 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with renal failure caused by acute injury or hepatorenal syndrome have classically not been included as candidates for combined transplantation because of the reversibility of renal dysfunction after liver transplantation .
	manualset3
121969	6	404971	5	NULL	NULL	0	NULL	combined transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with renal failure caused by acute injury or hepatorenal syndrome have classically not been included as candidates for combined transplantation because of the reversibility of renal dysfunction after liver transplantation .
	manualset3
121970	7	404971	5	NULL	NULL	0	NULL	renal dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with renal failure caused by acute injury or hepatorenal syndrome have classically not been included as candidates for combined transplantation because of the reversibility of renal dysfunction after liver transplantation .
	manualset3
121971	8	404971	5	NULL	NULL	0	NULL	liver transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with renal failure caused by acute injury or hepatorenal syndrome have classically not been included as candidates for combined transplantation because of the reversibility of renal dysfunction after liver transplantation .
	manualset3
121972	1	404972	5	NULL	NULL	0	NULL	genome scan	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A genome scan showed the presence of polymorphic alleles on chromosomes 2 , 6 , 7 and 15 with significant effects on body weight at 2-4 months , at 10-12 months , or at both age ranges , showing that weight gain trajectory in this stock is under complex genetic control .
	manualset3
121973	2	404972	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A genome scan showed the presence of polymorphic alleles on chromosomes 2 , 6 , 7 and 15 with significant effects on body weight at 2-4 months , at 10-12 months , or at both age ranges , showing that weight gain trajectory in this stock is under complex genetic control .
	manualset3
121974	3	404972	5	NULL	NULL	0	NULL	polymorphic alleles	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A genome scan showed the presence of polymorphic alleles on chromosomes 2 , 6 , 7 and 15 with significant effects on body weight at 2-4 months , at 10-12 months , or at both age ranges , showing that weight gain trajectory in this stock is under complex genetic control .
	manualset3
121975	4	404972	5	NULL	NULL	0	NULL	chromosome 2	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	A genome scan showed the presence of polymorphic alleles on chromosomes 2 , 6 , 7 and 15 with significant effects on body weight at 2-4 months , at 10-12 months , or at both age ranges , showing that weight gain trajectory in this stock is under complex genetic control .
	manualset3
121976	5	404972	5	NULL	NULL	NULL	NULL	chromosome 6	Chromosome												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A genome scan showed the presence of polymorphic alleles on chromosomes 2 , 6 , 7 and 15 with significant effects on body weight at 2-4 months , at 10-12 months , or at both age ranges , showing that weight gain trajectory in this stock is under complex genetic control .
	manualset3
121977	6	404972	5	NULL	NULL	0	NULL	chromosome 7	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	A genome scan showed the presence of polymorphic alleles on chromosomes 2 , 6 , 7 and 15 with significant effects on body weight at 2-4 months , at 10-12 months , or at both age ranges , showing that weight gain trajectory in this stock is under complex genetic control .
	manualset3
121978	7	404972	5	NULL	NULL	0	NULL	chromosome 15	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	A genome scan showed the presence of polymorphic alleles on chromosomes 2 , 6 , 7 and 15 with significant effects on body weight at 2-4 months , at 10-12 months , or at both age ranges , showing that weight gain trajectory in this stock is under complex genetic control .
	manualset3
121979	8	404972	5	NULL	NULL	0	NULL	significant effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A genome scan showed the presence of polymorphic alleles on chromosomes 2 , 6 , 7 and 15 with significant effects on body weight at 2-4 months , at 10-12 months , or at both age ranges , showing that weight gain trajectory in this stock is under complex genetic control .
	manualset3
121980	9	404972	5	NULL	NULL	0	NULL	body weight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A genome scan showed the presence of polymorphic alleles on chromosomes 2 , 6 , 7 and 15 with significant effects on body weight at 2-4 months , at 10-12 months , or at both age ranges , showing that weight gain trajectory in this stock is under complex genetic control .
	manualset3
121981	10	404972	5	NULL	NULL	NULL	NULL	2-4 months	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A genome scan showed the presence of polymorphic alleles on chromosomes 2 , 6 , 7 and 15 with significant effects on body weight at 2-4 months , at 10-12 months , or at both age ranges , showing that weight gain trajectory in this stock is under complex genetic control .
	manualset3
121982	11	404972	5	NULL	NULL	0	NULL	 10-12 months	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	A genome scan showed the presence of polymorphic alleles on chromosomes 2 , 6 , 7 and 15 with significant effects on body weight at 2-4 months , at 10-12 months , or at both age ranges , showing that weight gain trajectory in this stock is under complex genetic control .
	manualset3
121983	12	404972	5	NULL	NULL	0	NULL	age ranges	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A genome scan showed the presence of polymorphic alleles on chromosomes 2 , 6 , 7 and 15 with significant effects on body weight at 2-4 months , at 10-12 months , or at both age ranges , showing that weight gain trajectory in this stock is under complex genetic control .
	manualset3
121985	13	404972	5	NULL	NULL	0	NULL	weight gain trajectory 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A genome scan showed the presence of polymorphic alleles on chromosomes 2 , 6 , 7 and 15 with significant effects on body weight at 2-4 months , at 10-12 months , or at both age ranges , showing that weight gain trajectory in this stock is under complex genetic control .
	manualset3
121986	14	404972	5	NULL	NULL	0	NULL	stock 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A genome scan showed the presence of polymorphic alleles on chromosomes 2 , 6 , 7 and 15 with significant effects on body weight at 2-4 months , at 10-12 months , or at both age ranges , showing that weight gain trajectory in this stock is under complex genetic control .
	manualset3
121987	15	404972	5	NULL	NULL	0	NULL	complex genetic control	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A genome scan showed the presence of polymorphic alleles on chromosomes 2 , 6 , 7 and 15 with significant effects on body weight at 2-4 months , at 10-12 months , or at both age ranges , showing that weight gain trajectory in this stock is under complex genetic control .
	manualset3
121988	1	404973	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with sickle cell anemia in the New World probably correspond to various combinations of these types , in addition to the still hematologically undefined haplotype associated with sickle cell anemia in the Bantu-speaking areas of Africa .
	manualset3
121989	2	404973	5	NULL	NULL	0	NULL	sickle cell anemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with sickle cell anemia in the New World probably correspond to various combinations of these types , in addition to the still hematologically undefined haplotype associated with sickle cell anemia in the Bantu-speaking areas of Africa .
	manualset3
121990	3	404973	5	NULL	NULL	0	NULL	New World 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with sickle cell anemia in the New World probably correspond to various combinations of these types , in addition to the still hematologically undefined haplotype associated with sickle cell anemia in the Bantu-speaking areas of Africa .
	manualset3
121991	4	404973	5	NULL	NULL	0	NULL	combinations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with sickle cell anemia in the New World probably correspond to various combinations of these types , in addition to the still hematologically undefined haplotype associated with sickle cell anemia in the Bantu-speaking areas of Africa .
	manualset3
121992	5	404973	5	NULL	NULL	0	NULL	types 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with sickle cell anemia in the New World probably correspond to various combinations of these types , in addition to the still hematologically undefined haplotype associated with sickle cell anemia in the Bantu-speaking areas of Africa .
	manualset3
121993	6	404973	5	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with sickle cell anemia in the New World probably correspond to various combinations of these types , in addition to the still hematologically undefined haplotype associated with sickle cell anemia in the Bantu-speaking areas of Africa .
	manualset3
121997	7	404973	5	NULL	NULL	0	NULL	hematologically undefined haplotype	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with sickle cell anemia in the New World probably correspond to various combinations of these types , in addition to the still hematologically undefined haplotype associated with sickle cell anemia in the Bantu-speaking areas of Africa .
	manualset3
121999	8	404973	5	NULL	NULL	0	NULL	sickle cell anemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with sickle cell anemia in the New World probably correspond to various combinations of these types , in addition to the still hematologically undefined haplotype associated with sickle cell anemia in the Bantu-speaking areas of Africa .
	manualset3
122000	9	404973	5	NULL	NULL	0	NULL	Bantu-speaking areas of Africa	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with sickle cell anemia in the New World probably correspond to various combinations of these types , in addition to the still hematologically undefined haplotype associated with sickle cell anemia in the Bantu-speaking areas of Africa .
	manualset3
122001	1	404974	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with such mutations could behave differently than patients with IPD with respect to MIBG cardiac uptake and olfaction .
	manualset3
122002	2	404974	5	NULL	NULL	0	NULL	mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with such mutations could behave differently than patients with IPD with respect to MIBG cardiac uptake and olfaction .
	manualset3
122009	3	404974	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with such mutations could behave differently than patients with IPD with respect to MIBG cardiac uptake and olfaction .
	manualset3
122013	4	404974	5	NULL	NULL	0	NULL	IPD 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with such mutations could behave differently than patients with IPD with respect to MIBG cardiac uptake and olfaction .
	manualset3
122014	5	404974	5	NULL	NULL	0	NULL	MIBG cardiac uptake 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with such mutations could behave differently than patients with IPD with respect to MIBG cardiac uptake and olfaction .
	manualset3
122015	6	404974	5	NULL	NULL	0	NULL	olfaction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with such mutations could behave differently than patients with IPD with respect to MIBG cardiac uptake and olfaction .
	manualset3
122016	1	404975	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with the WHO-defined metabolic syndrome had an increased risk of having higher coronary-artery calcification scores , independent of age and sex ( OR = 2.02 , 95 % CI : 1.03-3 .97 , P = 0.04 ) .
	manualset3
122017	2	404975	5	NULL	NULL	0	NULL	WHO-defined metabolic syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with the WHO-defined metabolic syndrome had an increased risk of having higher coronary-artery calcification scores , independent of age and sex ( OR = 2.02 , 95 % CI : 1.03-3 .97 , P = 0.04 ) .
	manualset3
122018	3	404975	5	NULL	NULL	0	NULL	increased risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with the WHO-defined metabolic syndrome had an increased risk of having higher coronary-artery calcification scores , independent of age and sex ( OR = 2.02 , 95 % CI : 1.03-3 .97 , P = 0.04 ) .
	manualset3
122019	4	404975	5	NULL	NULL	0	NULL	coronary-artery calcification scores 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with the WHO-defined metabolic syndrome had an increased risk of having higher coronary-artery calcification scores , independent of age and sex ( OR = 2.02 , 95 % CI : 1.03-3 .97 , P = 0.04 ) .
	manualset3
122022	5	404975	5	NULL	NULL	0	NULL	age 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with the WHO-defined metabolic syndrome had an increased risk of having higher coronary-artery calcification scores , independent of age and sex ( OR = 2.02 , 95 % CI : 1.03-3 .97 , P = 0.04 ) .
	manualset3
122023	6	404975	5	NULL	NULL	0	NULL	sex 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with the WHO-defined metabolic syndrome had an increased risk of having higher coronary-artery calcification scores , independent of age and sex ( OR = 2.02 , 95 % CI : 1.03-3 .97 , P = 0.04 ) .
	manualset3
122024	7	404975	5	NULL	NULL	0	NULL	OR = 2.02 , 95 % CI : 1.03-3 .97 , P = 0.04 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with the WHO-defined metabolic syndrome had an increased risk of having higher coronary-artery calcification scores , independent of age and sex ( OR = 2.02 , 95 % CI : 1.03-3 .97 , P = 0.04 ) .
	manualset3
122025	1	404976	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with this disorder generally have minimal symptoms despite complete absence of the most abundant serum protein .
	manualset3
122026	2	404976	5	NULL	NULL	0	NULL	disorder 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with this disorder generally have minimal symptoms despite complete absence of the most abundant serum protein .
	manualset3
122028	3	404976	5	NULL	NULL	0	NULL	minimal symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with this disorder generally have minimal symptoms despite complete absence of the most abundant serum protein .
	manualset3
122030	4	404976	5	NULL	NULL	0	NULL	absence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with this disorder generally have minimal symptoms despite complete absence of the most abundant serum protein .
	manualset3
122033	5	404976	5	NULL	NULL	0	NULL	serum protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with this disorder generally have minimal symptoms despite complete absence of the most abundant serum protein .
	manualset3
122034	1	404977	5	NULL	NULL	0	NULL	Patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with tumors expressing Prx2 had better prognosis ( p = 0.027 ) .
	manualset3
122035	2	404977	5	NULL	NULL	0	NULL	tumors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with tumors expressing Prx2 had better prognosis ( p = 0.027 ) .
	manualset3
122036	3	404977	5	NULL	NULL	0	NULL	 Prx2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with tumors expressing Prx2 had better prognosis ( p = 0.027 ) .
	manualset3
122038	4	404977	5	NULL	NULL	0	NULL	prognosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with tumors expressing Prx2 had better prognosis ( p = 0.027 ) .
	manualset3
122043	5	404977	5	NULL	NULL	0	NULL	 p = 0.027	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with tumors expressing Prx2 had better prognosis ( p = 0.027 ) .
	manualset3
122046	1	404978	5	NULL	NULL	0	NULL	germline substitution 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A germline substitution in the human MSH2 gene is associated with high-grade dysplasia and cancer in ulcerative colitis .
	manualset3
122047	2	404978	5	NULL	NULL	0	NULL	human MSH2 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A germline substitution in the human MSH2 gene is associated with high-grade dysplasia and cancer in ulcerative colitis .
	manualset3
122048	3	404978	5	NULL	NULL	0	NULL	high-grade dysplasia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A germline substitution in the human MSH2 gene is associated with high-grade dysplasia and cancer in ulcerative colitis .
	manualset3
122049	4	404978	5	NULL	NULL	0	NULL	cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A germline substitution in the human MSH2 gene is associated with high-grade dysplasia and cancer in ulcerative colitis .
	manualset3
122050	5	404978	5	NULL	NULL	0	NULL	ulcerative colitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A germline substitution in the human MSH2 gene is associated with high-grade dysplasia and cancer in ulcerative colitis .
	manualset3
122051	1	404979	5	NULL	NULL	0	NULL	Patulin production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Patulin production was stimulated when the temperature decreased ( from 20 to 10 or 4 degrees C ) , while a further decrease of the temperature to 1 degrees C caused a reduction in patulin production .
	manualset3
122052	2	404979	5	NULL	NULL	0	NULL	temperature 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patulin production was stimulated when the temperature decreased ( from 20 to 10 or 4 degrees C ) , while a further decrease of the temperature to 1 degrees C caused a reduction in patulin production .
	manualset3
122053	3	404979	5	NULL	NULL	0	NULL	 20 to 10 or 4 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patulin production was stimulated when the temperature decreased ( from 20 to 10 or 4 degrees C ) , while a further decrease of the temperature to 1 degrees C caused a reduction in patulin production .
	manualset3
122054	4	404979	5	NULL	NULL	0	NULL	decrease 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patulin production was stimulated when the temperature decreased ( from 20 to 10 or 4 degrees C ) , while a further decrease of the temperature to 1 degrees C caused a reduction in patulin production .
	manualset3
122055	5	404979	5	NULL	NULL	0	NULL	temperature 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patulin production was stimulated when the temperature decreased ( from 20 to 10 or 4 degrees C ) , while a further decrease of the temperature to 1 degrees C caused a reduction in patulin production .
	manualset3
122056	6	404979	5	NULL	NULL	0	NULL	1 degrees C 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Patulin production was stimulated when the temperature decreased ( from 20 to 10 or 4 degrees C ) , while a further decrease of the temperature to 1 degrees C caused a reduction in patulin production .
	manualset3
122057	7	404979	5	NULL	NULL	0	NULL	reduction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patulin production was stimulated when the temperature decreased ( from 20 to 10 or 4 degrees C ) , while a further decrease of the temperature to 1 degrees C caused a reduction in patulin production .
	manualset3
122058	8	404979	5	NULL	NULL	0	NULL	patulin production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Patulin production was stimulated when the temperature decreased ( from 20 to 10 or 4 degrees C ) , while a further decrease of the temperature to 1 degrees C caused a reduction in patulin production .
	manualset3
122059	1	404980	5	NULL	NULL	0	NULL	strategic locations	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pausing at strategic locations may be a general mechanism for coordinated folding and conformational rearrangements of riboswitch structures that underlie their response to environmental cues .
	manualset3
122060	2	404980	5	NULL	NULL	0	NULL	general mechanism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pausing at strategic locations may be a general mechanism for coordinated folding and conformational rearrangements of riboswitch structures that underlie their response to environmental cues .
	manualset3
122062	3	404980	5	NULL	NULL	0	NULL	coordinated folding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pausing at strategic locations may be a general mechanism for coordinated folding and conformational rearrangements of riboswitch structures that underlie their response to environmental cues .
	manualset3
122063	4	404980	5	NULL	NULL	0	NULL	conformational rearrangements	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pausing at strategic locations may be a general mechanism for coordinated folding and conformational rearrangements of riboswitch structures that underlie their response to environmental cues .
	manualset3
122066	5	404980	5	NULL	NULL	0	NULL	riboswitch structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pausing at strategic locations may be a general mechanism for coordinated folding and conformational rearrangements of riboswitch structures that underlie their response to environmental cues .
	manualset3
122067	6	404980	5	NULL	NULL	0	NULL	response 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pausing at strategic locations may be a general mechanism for coordinated folding and conformational rearrangements of riboswitch structures that underlie their response to environmental cues .
	manualset3
122068	7	404980	5	NULL	NULL	0	NULL	environmental cues	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pausing at strategic locations may be a general mechanism for coordinated folding and conformational rearrangements of riboswitch structures that underlie their response to environmental cues .
	manualset3
122069	1	404981	5	NULL	NULL	0	NULL	Pax-6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Pax-6 is also expressed in the developing eye , the pituitary and the nasal epithelium .
	manualset3
122071	2	404981	5	NULL	NULL	0	NULL	developing eye	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Pax-6 is also expressed in the developing eye , the pituitary and the nasal epithelium .
	manualset3
122073	3	404981	5	NULL	NULL	0	NULL	pituitary 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Pax-6 is also expressed in the developing eye , the pituitary and the nasal epithelium .
	manualset3
122074	4	404981	5	NULL	NULL	0	NULL	nasal epithelium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Pax-6 is also expressed in the developing eye , the pituitary and the nasal epithelium .
	manualset3
122076	1	404982	5	NULL	NULL	0	NULL	Peak hair codeine concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Peak hair codeine concentrations for the 5 - , 10 - , and 20-mg/kg groups occurred 20 days after beginning the dosing protocol and were 0.57 + / - 0.13 , 0.80 + / - 0.10 , and 1.95 + / - 0.35 ng/mg hair , respectively .
	manualset3
122078	2	404982	5	NULL	NULL	0	NULL	5 -mg/kg groups 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Peak hair codeine concentrations for the 5 - , 10 - , and 20-mg/kg groups occurred 20 days after beginning the dosing protocol and were 0.57 + / - 0.13 , 0.80 + / - 0.10 , and 1.95 + / - 0.35 ng/mg hair , respectively .
	manualset3
122079	3	404982	5	NULL	NULL	0	NULL	10 -mg/kg groups 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Peak hair codeine concentrations for the 5 - , 10 - , and 20-mg/kg groups occurred 20 days after beginning the dosing protocol and were 0.57 + / - 0.13 , 0.80 + / - 0.10 , and 1.95 + / - 0.35 ng/mg hair , respectively .
	manualset3
122080	4	404982	5	NULL	NULL	0	NULL	20-mg/kg groups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Peak hair codeine concentrations for the 5 - , 10 - , and 20-mg/kg groups occurred 20 days after beginning the dosing protocol and were 0.57 + / - 0.13 , 0.80 + / - 0.10 , and 1.95 + / - 0.35 ng/mg hair , respectively .
	manualset3
122081	5	404982	5	NULL	NULL	0	NULL	20 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Peak hair codeine concentrations for the 5 - , 10 - , and 20-mg/kg groups occurred 20 days after beginning the dosing protocol and were 0.57 + / - 0.13 , 0.80 + / - 0.10 , and 1.95 + / - 0.35 ng/mg hair , respectively .
	manualset3
122082	6	404982	5	NULL	NULL	0	NULL	dosing protocol	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Peak hair codeine concentrations for the 5 - , 10 - , and 20-mg/kg groups occurred 20 days after beginning the dosing protocol and were 0.57 + / - 0.13 , 0.80 + / - 0.10 , and 1.95 + / - 0.35 ng/mg hair , respectively .
	manualset3
122083	7	404982	5	NULL	NULL	0	NULL	 0.57 + / - 0.13 ng/mg hair	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Peak hair codeine concentrations for the 5 - , 10 - , and 20-mg/kg groups occurred 20 days after beginning the dosing protocol and were 0.57 + / - 0.13 , 0.80 + / - 0.10 , and 1.95 + / - 0.35 ng/mg hair , respectively .
	manualset3
122090	8	404982	5	NULL	NULL	0	NULL	0.80 + / - 0.10 ng/mg hair	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Peak hair codeine concentrations for the 5 - , 10 - , and 20-mg/kg groups occurred 20 days after beginning the dosing protocol and were 0.57 + / - 0.13 , 0.80 + / - 0.10 , and 1.95 + / - 0.35 ng/mg hair , respectively .
	manualset3
122091	9	404982	5	NULL	NULL	0	NULL	1.95 + / - 0.35 ng/mg hair	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Peak hair codeine concentrations for the 5 - , 10 - , and 20-mg/kg groups occurred 20 days after beginning the dosing protocol and were 0.57 + / - 0.13 , 0.80 + / - 0.10 , and 1.95 + / - 0.35 ng/mg hair , respectively .
	manualset3
122092	1	404983	5	NULL	NULL	0	NULL	Peak time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Peak time was significantly earlier and peak level significantly higher in serum for syrup as compared to tablet .
	manualset3
122095	2	404983	5	NULL	NULL	0	NULL	peak level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Peak time was significantly earlier and peak level significantly higher in serum for syrup as compared to tablet .
	manualset3
122096	3	404983	5	NULL	NULL	0	NULL	serum 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Peak time was significantly earlier and peak level significantly higher in serum for syrup as compared to tablet .
	manualset3
122097	4	404983	5	NULL	NULL	0	NULL	syrup 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Peak time was significantly earlier and peak level significantly higher in serum for syrup as compared to tablet .
	manualset3
122098	5	404983	5	NULL	NULL	0	NULL	tablet 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Peak time was significantly earlier and peak level significantly higher in serum for syrup as compared to tablet .
	manualset3
122109	1	404984	5	NULL	NULL	0	NULL	global baseline	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A global baseline for spawning aggregations of reef fishes .
	manualset3
122110	2	404984	5	NULL	NULL	0	NULL	spawning aggregations 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A global baseline for spawning aggregations of reef fishes .
	manualset3
122111	3	404984	5	NULL	NULL	0	NULL	reef fishes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A global baseline for spawning aggregations of reef fishes .
	manualset3
122112	1	404985	5	NULL	NULL	0	NULL	Peaks 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Peaks are identified as individual subseries elevated above the base line of duration n , all the points in which have magnitude at least G ( n ) , where the values of G are cut-off criteria based on the width of the peak .
	manualset3
122113	2	404985	5	NULL	NULL	0	NULL	individual subseries	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Peaks are identified as individual subseries elevated above the base line of duration n , all the points in which have magnitude at least G ( n ) , where the values of G are cut-off criteria based on the width of the peak .
	manualset3
122114	3	404985	5	NULL	NULL	0	NULL	base line	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Peaks are identified as individual subseries elevated above the base line of duration n , all the points in which have magnitude at least G ( n ) , where the values of G are cut-off criteria based on the width of the peak .
	manualset3
122115	4	404985	5	NULL	NULL	0	NULL	duration n	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Peaks are identified as individual subseries elevated above the base line of duration n , all the points in which have magnitude at least G ( n ) , where the values of G are cut-off criteria based on the width of the peak .
	manualset3
122116	5	404985	5	NULL	NULL	0	NULL	points 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Peaks are identified as individual subseries elevated above the base line of duration n , all the points in which have magnitude at least G ( n ) , where the values of G are cut-off criteria based on the width of the peak .
	manualset3
122117	6	404985	5	NULL	NULL	0	NULL	magnitude 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Peaks are identified as individual subseries elevated above the base line of duration n , all the points in which have magnitude at least G ( n ) , where the values of G are cut-off criteria based on the width of the peak .
	manualset3
122118	7	404985	5	NULL	NULL	0	NULL	G ( n ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Peaks are identified as individual subseries elevated above the base line of duration n , all the points in which have magnitude at least G ( n ) , where the values of G are cut-off criteria based on the width of the peak .
	manualset3
122119	8	404985	5	NULL	NULL	0	NULL	values 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Peaks are identified as individual subseries elevated above the base line of duration n , all the points in which have magnitude at least G ( n ) , where the values of G are cut-off criteria based on the width of the peak .
	manualset3
122120	9	404985	5	NULL	NULL	0	NULL	G	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Peaks are identified as individual subseries elevated above the base line of duration n , all the points in which have magnitude at least G ( n ) , where the values of G are cut-off criteria based on the width of the peak .
	manualset3
122121	10	404985	5	NULL	NULL	0	NULL	cut-off criteria	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Peaks are identified as individual subseries elevated above the base line of duration n , all the points in which have magnitude at least G ( n ) , where the values of G are cut-off criteria based on the width of the peak .
	manualset3
122122	11	404985	5	NULL	NULL	0	NULL	width 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Peaks are identified as individual subseries elevated above the base line of duration n , all the points in which have magnitude at least G ( n ) , where the values of G are cut-off criteria based on the width of the peak .
	manualset3
122123	12	404985	5	NULL	NULL	0	NULL	peak 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Peaks are identified as individual subseries elevated above the base line of duration n , all the points in which have magnitude at least G ( n ) , where the values of G are cut-off criteria based on the width of the peak .
	manualset3
122124	1	404986	5	NULL	NULL	0	NULL	Pearl onion	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pearl onion and leek ( A. ampeloprasum ) have higher relative amounts of methiin and propiin , respectively .
	manualset3
122125	2	404986	5	NULL	NULL	0	NULL	leek ( A. ampeloprasum )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pearl onion and leek ( A. ampeloprasum ) have higher relative amounts of methiin and propiin , respectively .
	manualset3
122126	3	404986	5	NULL	NULL	0	NULL	higher relative amounts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pearl onion and leek ( A. ampeloprasum ) have higher relative amounts of methiin and propiin , respectively .
	manualset3
122127	4	404986	5	NULL	NULL	0	NULL	methiin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Pearl onion and leek ( A. ampeloprasum ) have higher relative amounts of methiin and propiin , respectively .
	manualset3
122128	5	404986	5	NULL	NULL	0	NULL	propiin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Pearl onion and leek ( A. ampeloprasum ) have higher relative amounts of methiin and propiin , respectively .
	manualset3
122129	1	404987	5	NULL	NULL	NULL	NULL	Pediatric residents ' ability	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pediatric residents ' ability to perform a lumbar puncture : evaluation of an educational intervention .
	manualset3
122132	2	404987	5	NULL	NULL	0	NULL	lumbar puncture	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pediatric residents ' ability to perform a lumbar puncture : evaluation of an educational intervention .
	manualset3
122135	3	404987	5	NULL	NULL	0	NULL	evaluation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pediatric residents ' ability to perform a lumbar puncture : evaluation of an educational intervention .
	manualset3
122137	4	404987	5	NULL	NULL	0	NULL	educational intervention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pediatric residents ' ability to perform a lumbar puncture : evaluation of an educational intervention .
	manualset3
122139	1	404988	5	NULL	NULL	0	NULL	barriers 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Peering through the barriers in GPs ' explanations for declining to participate in research : the role of professional autonomy and the economy of time .
	manualset3
122140	2	404988	5	NULL	NULL	0	NULL	GPs	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Peering through the barriers in GPs ' explanations for declining to participate in research : the role of professional autonomy and the economy of time .
	manualset3
122235	3	404988	5	NULL	NULL	0	NULL	explanations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Peering through the barriers in GPs ' explanations for declining to participate in research : the role of professional autonomy and the economy of time .
	manualset3
122237	5	404988	5	NULL	NULL	0	NULL	research 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Peering through the barriers in GPs ' explanations for declining to participate in research : the role of professional autonomy and the economy of time .
	manualset3
122238	6	404988	5	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Peering through the barriers in GPs ' explanations for declining to participate in research : the role of professional autonomy and the economy of time .
	manualset3
122239	7	404988	5	NULL	NULL	0	NULL	professional autonomy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Peering through the barriers in GPs ' explanations for declining to participate in research : the role of professional autonomy and the economy of time .
	manualset3
122240	8	404988	5	NULL	NULL	0	NULL	economy 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Peering through the barriers in GPs ' explanations for declining to participate in research : the role of professional autonomy and the economy of time .
	manualset3
122241	9	404988	5	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Peering through the barriers in GPs ' explanations for declining to participate in research : the role of professional autonomy and the economy of time .
	manualset3
122242	1	404989	5	NULL	NULL	0	NULL	Pelvic haemangiopericytoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pelvic haemangiopericytoma : preoperative arteriographic demonstration .
	manualset3
122243	2	404989	5	NULL	NULL	0	NULL	preoperative arteriographic demonstration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pelvic haemangiopericytoma : preoperative arteriographic demonstration .
	manualset3
122244	1	404990	5	NULL	NULL	0	NULL	Pelvic measurement 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pelvic measurement can be included in evaluation of UI .
	manualset3
122245	2	404990	5	NULL	NULL	0	NULL	evaluation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pelvic measurement can be included in evaluation of UI .
	manualset3
122246	3	404990	5	NULL	NULL	0	NULL	UI 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pelvic measurement can be included in evaluation of UI .
	manualset3
122247	1	404991	5	NULL	NULL	0	NULL	global role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A global role for KLF1 in erythropoiesis revealed by ChIP-seq in primary erythroid cells .
	manualset3
122248	2	404991	5	NULL	NULL	0	NULL	KLF1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A global role for KLF1 in erythropoiesis revealed by ChIP-seq in primary erythroid cells .
	manualset3
122249	3	404991	5	NULL	NULL	0	NULL	erythropoiesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A global role for KLF1 in erythropoiesis revealed by ChIP-seq in primary erythroid cells .
	manualset3
122250	4	404991	5	NULL	NULL	0	NULL	ChIP-seq	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A global role for KLF1 in erythropoiesis revealed by ChIP-seq in primary erythroid cells .
	manualset3
122251	5	404991	5	NULL	NULL	0	NULL	primary erythroid cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A global role for KLF1 in erythropoiesis revealed by ChIP-seq in primary erythroid cells .
	manualset3
122304	1	404992	5	NULL	NULL	0	NULL	Pemphigus antigens	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Pemphigus and pemphigoid antigens are expressed in human amnion epithelium .
	manualset3
122305	2	404992	5	NULL	NULL	0	NULL	pemphigoid antigens 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Pemphigus and pemphigoid antigens are expressed in human amnion epithelium .
	manualset3
122306	3	404992	5	NULL	NULL	0	NULL	human amnion epithelium	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Pemphigus and pemphigoid antigens are expressed in human amnion epithelium .
	manualset3
122307	1	404993	5	NULL	NULL	0	NULL	Pemphigus vulgaris ( PV )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pemphigus vulgaris ( PV ) is a Th2-dominant autoimmune skin disease .
	manualset3
122308	2	404993	5	NULL	NULL	0	NULL	Th2-dominant autoimmune skin disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pemphigus vulgaris ( PV ) is a Th2-dominant autoimmune skin disease .
	manualset3
122309	1	404994	5	NULL	NULL	0	NULL	wounds 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Penetrating wounds were present in only two cases ( 15 % ) , the other patients ( 85 % ) were affected by blunt trauma .
	manualset3
122310	2	404994	5	NULL	NULL	0	NULL	two cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Penetrating wounds were present in only two cases ( 15 % ) , the other patients ( 85 % ) were affected by blunt trauma .
	manualset3
122311	3	404994	5	NULL	NULL	0	NULL	15 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Penetrating wounds were present in only two cases ( 15 % ) , the other patients ( 85 % ) were affected by blunt trauma .
	manualset3
122312	4	404994	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Penetrating wounds were present in only two cases ( 15 % ) , the other patients ( 85 % ) were affected by blunt trauma .
	manualset3
122313	5	404994	5	NULL	NULL	0	NULL	85 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Penetrating wounds were present in only two cases ( 15 % ) , the other patients ( 85 % ) were affected by blunt trauma .
	manualset3
122314	6	404994	5	NULL	NULL	0	NULL	blunt trauma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Penetrating wounds were present in only two cases ( 15 % ) , the other patients ( 85 % ) were affected by blunt trauma .
	manualset3
122315	1	404995	5	NULL	NULL	0	NULL	Pentazocine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pentazocine , butorphanol , nalbuphine , and buprenorphine are mixed agonist-antagonist opioids that are effective analgesics , with less abuse potential than the agonists morphine , propoxyphene , and codeine .
	manualset3
122316	2	404995	5	NULL	NULL	0	NULL	butorphanol 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pentazocine , butorphanol , nalbuphine , and buprenorphine are mixed agonist-antagonist opioids that are effective analgesics , with less abuse potential than the agonists morphine , propoxyphene , and codeine .
	manualset3
122317	3	404995	5	NULL	NULL	0	NULL	nalbuphine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pentazocine , butorphanol , nalbuphine , and buprenorphine are mixed agonist-antagonist opioids that are effective analgesics , with less abuse potential than the agonists morphine , propoxyphene , and codeine .
	manualset3
122318	4	404995	5	NULL	NULL	0	NULL	buprenorphine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pentazocine , butorphanol , nalbuphine , and buprenorphine are mixed agonist-antagonist opioids that are effective analgesics , with less abuse potential than the agonists morphine , propoxyphene , and codeine .
	manualset3
122319	5	404995	5	NULL	NULL	0	NULL	agonist-antagonist opioids	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pentazocine , butorphanol , nalbuphine , and buprenorphine are mixed agonist-antagonist opioids that are effective analgesics , with less abuse potential than the agonists morphine , propoxyphene , and codeine .
	manualset3
122320	6	404995	5	NULL	NULL	0	NULL	analgesics 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pentazocine , butorphanol , nalbuphine , and buprenorphine are mixed agonist-antagonist opioids that are effective analgesics , with less abuse potential than the agonists morphine , propoxyphene , and codeine .
	manualset3
122321	7	404995	5	NULL	NULL	0	NULL	abuse potential 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pentazocine , butorphanol , nalbuphine , and buprenorphine are mixed agonist-antagonist opioids that are effective analgesics , with less abuse potential than the agonists morphine , propoxyphene , and codeine .
	manualset3
122322	8	404995	5	NULL	NULL	0	NULL	morphine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pentazocine , butorphanol , nalbuphine , and buprenorphine are mixed agonist-antagonist opioids that are effective analgesics , with less abuse potential than the agonists morphine , propoxyphene , and codeine .
	manualset3
122323	9	404995	5	NULL	NULL	0	NULL	propoxyphene 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pentazocine , butorphanol , nalbuphine , and buprenorphine are mixed agonist-antagonist opioids that are effective analgesics , with less abuse potential than the agonists morphine , propoxyphene , and codeine .
	manualset3
122324	10	404995	5	NULL	NULL	0	NULL	codeine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pentazocine , butorphanol , nalbuphine , and buprenorphine are mixed agonist-antagonist opioids that are effective analgesics , with less abuse potential than the agonists morphine , propoxyphene , and codeine .
	manualset3
122325	1	404996	5	NULL	NULL	0	NULL	Pentazocine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pentazocine -- naloxone : another `` addiction-proof '' drug of abuse .
	manualset3
122326	2	404996	5	NULL	NULL	0	NULL	naloxone 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pentazocine -- naloxone : another `` addiction-proof '' drug of abuse .
	manualset3
122327	3	404996	5	NULL	NULL	0	NULL	drug 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pentazocine -- naloxone : another `` addiction-proof '' drug of abuse .
	manualset3
122328	4	404996	5	NULL	NULL	0	NULL	abuse 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pentazocine -- naloxone : another `` addiction-proof '' drug of abuse .
	manualset3
122329	1	404997	5	NULL	NULL	0	NULL	Pentobarbital 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pentobarbital markedly inhibited the mortality in these ischemic rats , whereas cyproheptadine did not .
	manualset3
122330	2	404997	5	NULL	NULL	0	NULL	mortality 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pentobarbital markedly inhibited the mortality in these ischemic rats , whereas cyproheptadine did not .
	manualset3
122331	3	404997	5	NULL	NULL	0	NULL	ischemic rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pentobarbital markedly inhibited the mortality in these ischemic rats , whereas cyproheptadine did not .
	manualset3
122332	4	404997	5	NULL	NULL	0	NULL	cyproheptadine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pentobarbital markedly inhibited the mortality in these ischemic rats , whereas cyproheptadine did not .
	manualset3
122333	1	404998	5	NULL	NULL	0	NULL	People 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	People in low awareness states following profound brain injury typically demonstrate subtle changes in functional behaviors which challenge the sensitivity of measurement tools .
	manualset3
122334	2	404998	5	NULL	NULL	0	NULL	low awareness states	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	People in low awareness states following profound brain injury typically demonstrate subtle changes in functional behaviors which challenge the sensitivity of measurement tools .
	manualset3
122335	3	404998	5	NULL	NULL	0	NULL	profound brain injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	People in low awareness states following profound brain injury typically demonstrate subtle changes in functional behaviors which challenge the sensitivity of measurement tools .
	manualset3
122336	4	404998	5	NULL	NULL	0	NULL	changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	People in low awareness states following profound brain injury typically demonstrate subtle changes in functional behaviors which challenge the sensitivity of measurement tools .
	manualset3
122337	5	404998	5	NULL	NULL	0	NULL	functional behaviors	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	People in low awareness states following profound brain injury typically demonstrate subtle changes in functional behaviors which challenge the sensitivity of measurement tools .
	manualset3
122338	6	404998	5	NULL	NULL	0	NULL	challenge 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	People in low awareness states following profound brain injury typically demonstrate subtle changes in functional behaviors which challenge the sensitivity of measurement tools .
	manualset3
122339	7	404998	5	NULL	NULL	0	NULL	sensitivity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	People in low awareness states following profound brain injury typically demonstrate subtle changes in functional behaviors which challenge the sensitivity of measurement tools .
	manualset3
122340	8	404998	5	NULL	NULL	0	NULL	measurement tools	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	People in low awareness states following profound brain injury typically demonstrate subtle changes in functional behaviors which challenge the sensitivity of measurement tools .
	manualset3
122341	1	404999	5	NULL	NULL	0	NULL	People 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	People working at the time of their interview in areas where they often handled dead , raw , unfrozen chickens were three times more likely to have developed warts ( Odds ratio ( OR ) = 3.0 , 95 % confidence interval ( CI ) : 1.2-8 .0 ) ; for those who had ever worked in these ` high-risk ' areas , this excess risk almost doubled ( OR = 5.6 , 95 % CI : 2.1-14 .7 ) .
	manualset3
122342	2	404999	5	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	People working at the time of their interview in areas where they often handled dead , raw , unfrozen chickens were three times more likely to have developed warts ( Odds ratio ( OR ) = 3.0 , 95 % confidence interval ( CI ) : 1.2-8 .0 ) ; for those who had ever worked in these ` high-risk ' areas , this excess risk almost doubled ( OR = 5.6 , 95 % CI : 2.1-14 .7 ) .
	manualset3
122343	3	404999	5	NULL	NULL	0	NULL	interview 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	People working at the time of their interview in areas where they often handled dead , raw , unfrozen chickens were three times more likely to have developed warts ( Odds ratio ( OR ) = 3.0 , 95 % confidence interval ( CI ) : 1.2-8 .0 ) ; for those who had ever worked in these ` high-risk ' areas , this excess risk almost doubled ( OR = 5.6 , 95 % CI : 2.1-14 .7 ) .
	manualset3
122344	4	404999	5	NULL	NULL	0	NULL	areas 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	People working at the time of their interview in areas where they often handled dead , raw , unfrozen chickens were three times more likely to have developed warts ( Odds ratio ( OR ) = 3.0 , 95 % confidence interval ( CI ) : 1.2-8 .0 ) ; for those who had ever worked in these ` high-risk ' areas , this excess risk almost doubled ( OR = 5.6 , 95 % CI : 2.1-14 .7 ) .
	manualset3
122345	5	404999	5	NULL	NULL	0	NULL	dead chickens 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	People working at the time of their interview in areas where they often handled dead , raw , unfrozen chickens were three times more likely to have developed warts ( Odds ratio ( OR ) = 3.0 , 95 % confidence interval ( CI ) : 1.2-8 .0 ) ; for those who had ever worked in these ` high-risk ' areas , this excess risk almost doubled ( OR = 5.6 , 95 % CI : 2.1-14 .7 ) .
	manualset3
122346	6	404999	5	NULL	NULL	0	NULL	 raw chickens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	People working at the time of their interview in areas where they often handled dead , raw , unfrozen chickens were three times more likely to have developed warts ( Odds ratio ( OR ) = 3.0 , 95 % confidence interval ( CI ) : 1.2-8 .0 ) ; for those who had ever worked in these ` high-risk ' areas , this excess risk almost doubled ( OR = 5.6 , 95 % CI : 2.1-14 .7 ) .
	manualset3
122347	7	404999	5	NULL	NULL	0	NULL	unfrozen chickens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	People working at the time of their interview in areas where they often handled dead , raw , unfrozen chickens were three times more likely to have developed warts ( Odds ratio ( OR ) = 3.0 , 95 % confidence interval ( CI ) : 1.2-8 .0 ) ; for those who had ever worked in these ` high-risk ' areas , this excess risk almost doubled ( OR = 5.6 , 95 % CI : 2.1-14 .7 ) .
	manualset3
122348	8	404999	5	NULL	NULL	0	NULL	three times	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	People working at the time of their interview in areas where they often handled dead , raw , unfrozen chickens were three times more likely to have developed warts ( Odds ratio ( OR ) = 3.0 , 95 % confidence interval ( CI ) : 1.2-8 .0 ) ; for those who had ever worked in these ` high-risk ' areas , this excess risk almost doubled ( OR = 5.6 , 95 % CI : 2.1-14 .7 ) .
	manualset3
122349	9	404999	5	NULL	NULL	0	NULL	warts 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	People working at the time of their interview in areas where they often handled dead , raw , unfrozen chickens were three times more likely to have developed warts ( Odds ratio ( OR ) = 3.0 , 95 % confidence interval ( CI ) : 1.2-8 .0 ) ; for those who had ever worked in these ` high-risk ' areas , this excess risk almost doubled ( OR = 5.6 , 95 % CI : 2.1-14 .7 ) .
	manualset3
122350	10	404999	5	NULL	NULL	0	NULL	 Odds ratio ( OR ) = 3.0 , 95 % confidence interval ( CI ) : 1.2-8 .0	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	People working at the time of their interview in areas where they often handled dead , raw , unfrozen chickens were three times more likely to have developed warts ( Odds ratio ( OR ) = 3.0 , 95 % confidence interval ( CI ) : 1.2-8 .0 ) ; for those who had ever worked in these ` high-risk ' areas , this excess risk almost doubled ( OR = 5.6 , 95 % CI : 2.1-14 .7 ) .
	manualset3
122351	11	404999	5	NULL	NULL	0	NULL	 ` high-risk ' areas	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	People working at the time of their interview in areas where they often handled dead , raw , unfrozen chickens were three times more likely to have developed warts ( Odds ratio ( OR ) = 3.0 , 95 % confidence interval ( CI ) : 1.2-8 .0 ) ; for those who had ever worked in these ` high-risk ' areas , this excess risk almost doubled ( OR = 5.6 , 95 % CI : 2.1-14 .7 ) .
	manualset3
122352	12	404999	5	NULL	NULL	0	NULL	risk 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	People working at the time of their interview in areas where they often handled dead , raw , unfrozen chickens were three times more likely to have developed warts ( Odds ratio ( OR ) = 3.0 , 95 % confidence interval ( CI ) : 1.2-8 .0 ) ; for those who had ever worked in these ` high-risk ' areas , this excess risk almost doubled ( OR = 5.6 , 95 % CI : 2.1-14 .7 ) .
	manualset3
122353	13	404999	5	NULL	NULL	0	NULL	 OR = 5.6 , 95 % CI : 2.1-14 .7	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	People working at the time of their interview in areas where they often handled dead , raw , unfrozen chickens were three times more likely to have developed warts ( Odds ratio ( OR ) = 3.0 , 95 % confidence interval ( CI ) : 1.2-8 .0 ) ; for those who had ever worked in these ` high-risk ' areas , this excess risk almost doubled ( OR = 5.6 , 95 % CI : 2.1-14 .7 ) .
	manualset3
122354	1	405000	5	NULL	NULL	NULL	NULL	Peptide inhibitors of alpha-amylase	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Peptide inhibitors of alpha-amylase based on tendamistat : development of analogs with omega-amino acids linking critical binding segments .
	manualset3
122355	2	405000	5	NULL	NULL	0	NULL	tendamistat 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptide inhibitors of alpha-amylase based on tendamistat : development of analogs with omega-amino acids linking critical binding segments .
	manualset3
122356	3	405000	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptide inhibitors of alpha-amylase based on tendamistat : development of analogs with omega-amino acids linking critical binding segments .
	manualset3
122357	4	405000	5	NULL	NULL	0	NULL	analogs 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptide inhibitors of alpha-amylase based on tendamistat : development of analogs with omega-amino acids linking critical binding segments .
	manualset3
122358	5	405000	5	NULL	NULL	0	NULL	omega-amino acids linking critical binding segments	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptide inhibitors of alpha-amylase based on tendamistat : development of analogs with omega-amino acids linking critical binding segments .
	manualset3
122409	1	405001	5	NULL	NULL	0	NULL	goal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A goal of this type of work is to make the designed system orthogonal , that is , able to function independently of systems in the host .
	manualset3
122410	2	405001	5	NULL	NULL	0	NULL	type 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A goal of this type of work is to make the designed system orthogonal , that is , able to function independently of systems in the host .
	manualset3
122411	3	405001	5	NULL	NULL	0	NULL	work 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A goal of this type of work is to make the designed system orthogonal , that is , able to function independently of systems in the host .
	manualset3
122412	4	405001	5	NULL	NULL	0	NULL	designed system	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A goal of this type of work is to make the designed system orthogonal , that is , able to function independently of systems in the host .
	manualset3
122414	6	405001	5	NULL	NULL	0	NULL	systems 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A goal of this type of work is to make the designed system orthogonal , that is , able to function independently of systems in the host .
	manualset3
122415	7	405001	5	NULL	NULL	0	NULL	host 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A goal of this type of work is to make the designed system orthogonal , that is , able to function independently of systems in the host .
	manualset3
122416	1	405002	5	NULL	NULL	0	NULL	Peptide phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptide phosphorylation occurs at both serine and threonine residues .
	manualset3
122417	2	405002	5	NULL	NULL	0	NULL	serine residue	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptide phosphorylation occurs at both serine and threonine residues .
	manualset3
122418	3	405002	5	NULL	NULL	0	NULL	threonine residue	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptide phosphorylation occurs at both serine and threonine residues .
	manualset3
122419	1	405003	5	NULL	NULL	0	NULL	Peptides 1-12	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptides 1-12 have the following substituents at position three in ( A ) : ( 1 ) Pro ; ( 2 ) Oic ; ( 3 ) Atc ; ( 4 ) D-Atc ; ( 6 ) D-Phe ; ( 7 ) Ile ; ( 8 ) Leu ; ( 9 ) Tyr ; ( 10 ) Trp ; ( 11 ) Hphe ; ( 12 ) ( HO ) Tic ; Peptide ( 13 ) is the Tyr-NH2 ( 9 ) analog of ( B ) : Peptide ( 14 ) is the D-Cys ( 6 ) analog of ( B ) .
	manualset3
122420	2	405003	5	NULL	NULL	0	NULL	substituents 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptides 1-12 have the following substituents at position three in ( A ) : ( 1 ) Pro ; ( 2 ) Oic ; ( 3 ) Atc ; ( 4 ) D-Atc ; ( 6 ) D-Phe ; ( 7 ) Ile ; ( 8 ) Leu ; ( 9 ) Tyr ; ( 10 ) Trp ; ( 11 ) Hphe ; ( 12 ) ( HO ) Tic ; Peptide ( 13 ) is the Tyr-NH2 ( 9 ) analog of ( B ) : Peptide ( 14 ) is the D-Cys ( 6 ) analog of ( B ) .
	manualset3
122421	3	405003	5	NULL	NULL	0	NULL	position three	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptides 1-12 have the following substituents at position three in ( A ) : ( 1 ) Pro ; ( 2 ) Oic ; ( 3 ) Atc ; ( 4 ) D-Atc ; ( 6 ) D-Phe ; ( 7 ) Ile ; ( 8 ) Leu ; ( 9 ) Tyr ; ( 10 ) Trp ; ( 11 ) Hphe ; ( 12 ) ( HO ) Tic ; Peptide ( 13 ) is the Tyr-NH2 ( 9 ) analog of ( B ) : Peptide ( 14 ) is the D-Cys ( 6 ) analog of ( B ) .
	manualset3
122422	4	405003	5	NULL	NULL	0	NULL	Pro 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptides 1-12 have the following substituents at position three in ( A ) : ( 1 ) Pro ; ( 2 ) Oic ; ( 3 ) Atc ; ( 4 ) D-Atc ; ( 6 ) D-Phe ; ( 7 ) Ile ; ( 8 ) Leu ; ( 9 ) Tyr ; ( 10 ) Trp ; ( 11 ) Hphe ; ( 12 ) ( HO ) Tic ; Peptide ( 13 ) is the Tyr-NH2 ( 9 ) analog of ( B ) : Peptide ( 14 ) is the D-Cys ( 6 ) analog of ( B ) .
	manualset3
122423	5	405003	5	NULL	NULL	0	NULL	Oic 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptides 1-12 have the following substituents at position three in ( A ) : ( 1 ) Pro ; ( 2 ) Oic ; ( 3 ) Atc ; ( 4 ) D-Atc ; ( 6 ) D-Phe ; ( 7 ) Ile ; ( 8 ) Leu ; ( 9 ) Tyr ; ( 10 ) Trp ; ( 11 ) Hphe ; ( 12 ) ( HO ) Tic ; Peptide ( 13 ) is the Tyr-NH2 ( 9 ) analog of ( B ) : Peptide ( 14 ) is the D-Cys ( 6 ) analog of ( B ) .
	manualset3
122424	6	405003	5	NULL	NULL	NULL	NULL	Atc 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Peptides 1-12 have the following substituents at position three in ( A ) : ( 1 ) Pro ; ( 2 ) Oic ; ( 3 ) Atc ; ( 4 ) D-Atc ; ( 6 ) D-Phe ; ( 7 ) Ile ; ( 8 ) Leu ; ( 9 ) Tyr ; ( 10 ) Trp ; ( 11 ) Hphe ; ( 12 ) ( HO ) Tic ; Peptide ( 13 ) is the Tyr-NH2 ( 9 ) analog of ( B ) : Peptide ( 14 ) is the D-Cys ( 6 ) analog of ( B ) .
	manualset3
122425	7	405003	5	NULL	NULL	0	NULL	D-Atc	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptides 1-12 have the following substituents at position three in ( A ) : ( 1 ) Pro ; ( 2 ) Oic ; ( 3 ) Atc ; ( 4 ) D-Atc ; ( 6 ) D-Phe ; ( 7 ) Ile ; ( 8 ) Leu ; ( 9 ) Tyr ; ( 10 ) Trp ; ( 11 ) Hphe ; ( 12 ) ( HO ) Tic ; Peptide ( 13 ) is the Tyr-NH2 ( 9 ) analog of ( B ) : Peptide ( 14 ) is the D-Cys ( 6 ) analog of ( B ) .
	manualset3
122426	8	405003	5	NULL	NULL	0	NULL	D-Phe	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptides 1-12 have the following substituents at position three in ( A ) : ( 1 ) Pro ; ( 2 ) Oic ; ( 3 ) Atc ; ( 4 ) D-Atc ; ( 6 ) D-Phe ; ( 7 ) Ile ; ( 8 ) Leu ; ( 9 ) Tyr ; ( 10 ) Trp ; ( 11 ) Hphe ; ( 12 ) ( HO ) Tic ; Peptide ( 13 ) is the Tyr-NH2 ( 9 ) analog of ( B ) : Peptide ( 14 ) is the D-Cys ( 6 ) analog of ( B ) .
	manualset3
122427	9	405003	5	NULL	NULL	0	NULL	Ile 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptides 1-12 have the following substituents at position three in ( A ) : ( 1 ) Pro ; ( 2 ) Oic ; ( 3 ) Atc ; ( 4 ) D-Atc ; ( 6 ) D-Phe ; ( 7 ) Ile ; ( 8 ) Leu ; ( 9 ) Tyr ; ( 10 ) Trp ; ( 11 ) Hphe ; ( 12 ) ( HO ) Tic ; Peptide ( 13 ) is the Tyr-NH2 ( 9 ) analog of ( B ) : Peptide ( 14 ) is the D-Cys ( 6 ) analog of ( B ) .
	manualset3
122428	10	405003	5	NULL	NULL	0	NULL	Leu 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptides 1-12 have the following substituents at position three in ( A ) : ( 1 ) Pro ; ( 2 ) Oic ; ( 3 ) Atc ; ( 4 ) D-Atc ; ( 6 ) D-Phe ; ( 7 ) Ile ; ( 8 ) Leu ; ( 9 ) Tyr ; ( 10 ) Trp ; ( 11 ) Hphe ; ( 12 ) ( HO ) Tic ; Peptide ( 13 ) is the Tyr-NH2 ( 9 ) analog of ( B ) : Peptide ( 14 ) is the D-Cys ( 6 ) analog of ( B ) .
	manualset3
122429	11	405003	5	NULL	NULL	0	NULL	Tyr 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptides 1-12 have the following substituents at position three in ( A ) : ( 1 ) Pro ; ( 2 ) Oic ; ( 3 ) Atc ; ( 4 ) D-Atc ; ( 6 ) D-Phe ; ( 7 ) Ile ; ( 8 ) Leu ; ( 9 ) Tyr ; ( 10 ) Trp ; ( 11 ) Hphe ; ( 12 ) ( HO ) Tic ; Peptide ( 13 ) is the Tyr-NH2 ( 9 ) analog of ( B ) : Peptide ( 14 ) is the D-Cys ( 6 ) analog of ( B ) .
	manualset3
122430	12	405003	5	NULL	NULL	0	NULL	Trp 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptides 1-12 have the following substituents at position three in ( A ) : ( 1 ) Pro ; ( 2 ) Oic ; ( 3 ) Atc ; ( 4 ) D-Atc ; ( 6 ) D-Phe ; ( 7 ) Ile ; ( 8 ) Leu ; ( 9 ) Tyr ; ( 10 ) Trp ; ( 11 ) Hphe ; ( 12 ) ( HO ) Tic ; Peptide ( 13 ) is the Tyr-NH2 ( 9 ) analog of ( B ) : Peptide ( 14 ) is the D-Cys ( 6 ) analog of ( B ) .
	manualset3
122431	13	405003	5	NULL	NULL	0	NULL	Hphe 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptides 1-12 have the following substituents at position three in ( A ) : ( 1 ) Pro ; ( 2 ) Oic ; ( 3 ) Atc ; ( 4 ) D-Atc ; ( 6 ) D-Phe ; ( 7 ) Ile ; ( 8 ) Leu ; ( 9 ) Tyr ; ( 10 ) Trp ; ( 11 ) Hphe ; ( 12 ) ( HO ) Tic ; Peptide ( 13 ) is the Tyr-NH2 ( 9 ) analog of ( B ) : Peptide ( 14 ) is the D-Cys ( 6 ) analog of ( B ) .
	manualset3
122436	14	405003	5	NULL	NULL	0	NULL	( HO ) Tic	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptides 1-12 have the following substituents at position three in ( A ) : ( 1 ) Pro ; ( 2 ) Oic ; ( 3 ) Atc ; ( 4 ) D-Atc ; ( 6 ) D-Phe ; ( 7 ) Ile ; ( 8 ) Leu ; ( 9 ) Tyr ; ( 10 ) Trp ; ( 11 ) Hphe ; ( 12 ) ( HO ) Tic ; Peptide ( 13 ) is the Tyr-NH2 ( 9 ) analog of ( B ) : Peptide ( 14 ) is the D-Cys ( 6 ) analog of ( B ) .
	manualset3
122437	15	405003	5	NULL	NULL	0	NULL	Peptide ( 13 ) 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptides 1-12 have the following substituents at position three in ( A ) : ( 1 ) Pro ; ( 2 ) Oic ; ( 3 ) Atc ; ( 4 ) D-Atc ; ( 6 ) D-Phe ; ( 7 ) Ile ; ( 8 ) Leu ; ( 9 ) Tyr ; ( 10 ) Trp ; ( 11 ) Hphe ; ( 12 ) ( HO ) Tic ; Peptide ( 13 ) is the Tyr-NH2 ( 9 ) analog of ( B ) : Peptide ( 14 ) is the D-Cys ( 6 ) analog of ( B ) .
	manualset3
122438	16	405003	5	NULL	NULL	0	NULL	Tyr-NH2 ( 9 ) analog	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptides 1-12 have the following substituents at position three in ( A ) : ( 1 ) Pro ; ( 2 ) Oic ; ( 3 ) Atc ; ( 4 ) D-Atc ; ( 6 ) D-Phe ; ( 7 ) Ile ; ( 8 ) Leu ; ( 9 ) Tyr ; ( 10 ) Trp ; ( 11 ) Hphe ; ( 12 ) ( HO ) Tic ; Peptide ( 13 ) is the Tyr-NH2 ( 9 ) analog of ( B ) : Peptide ( 14 ) is the D-Cys ( 6 ) analog of ( B ) .
	manualset3
122439	17	405003	5	NULL	NULL	0	NULL	Peptide ( 14 )	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptides 1-12 have the following substituents at position three in ( A ) : ( 1 ) Pro ; ( 2 ) Oic ; ( 3 ) Atc ; ( 4 ) D-Atc ; ( 6 ) D-Phe ; ( 7 ) Ile ; ( 8 ) Leu ; ( 9 ) Tyr ; ( 10 ) Trp ; ( 11 ) Hphe ; ( 12 ) ( HO ) Tic ; Peptide ( 13 ) is the Tyr-NH2 ( 9 ) analog of ( B ) : Peptide ( 14 ) is the D-Cys ( 6 ) analog of ( B ) .
	manualset3
122440	18	405003	5	NULL	NULL	0	NULL	D-Cys ( 6 ) analog	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptides 1-12 have the following substituents at position three in ( A ) : ( 1 ) Pro ; ( 2 ) Oic ; ( 3 ) Atc ; ( 4 ) D-Atc ; ( 6 ) D-Phe ; ( 7 ) Ile ; ( 8 ) Leu ; ( 9 ) Tyr ; ( 10 ) Trp ; ( 11 ) Hphe ; ( 12 ) ( HO ) Tic ; Peptide ( 13 ) is the Tyr-NH2 ( 9 ) analog of ( B ) : Peptide ( 14 ) is the D-Cys ( 6 ) analog of ( B ) .
	manualset3
122441	1	405004	5	NULL	NULL	0	NULL	Peptides 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptides were synthesized that correspond to the antigenic sequences from ovalbumin and influenza nucleoprotein believed to be naturally processed and presented by cells with Kb and Db MHC class I molecules , respectively .
	manualset3
122442	2	405004	5	NULL	NULL	0	NULL	antigenic sequences	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptides were synthesized that correspond to the antigenic sequences from ovalbumin and influenza nucleoprotein believed to be naturally processed and presented by cells with Kb and Db MHC class I molecules , respectively .
	manualset3
122443	3	405004	5	NULL	NULL	0	NULL	ovalbumin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptides were synthesized that correspond to the antigenic sequences from ovalbumin and influenza nucleoprotein believed to be naturally processed and presented by cells with Kb and Db MHC class I molecules , respectively .
	manualset3
122444	4	405004	5	NULL	NULL	0	NULL	influenza nucleoprotein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptides were synthesized that correspond to the antigenic sequences from ovalbumin and influenza nucleoprotein believed to be naturally processed and presented by cells with Kb and Db MHC class I molecules , respectively .
	manualset3
122445	5	405004	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptides were synthesized that correspond to the antigenic sequences from ovalbumin and influenza nucleoprotein believed to be naturally processed and presented by cells with Kb and Db MHC class I molecules , respectively .
	manualset3
122473	6	405004	5	NULL	NULL	0	NULL	Kb MHC class I molecules 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptides were synthesized that correspond to the antigenic sequences from ovalbumin and influenza nucleoprotein believed to be naturally processed and presented by cells with Kb and Db MHC class I molecules , respectively .
	manualset3
122475	7	405004	5	NULL	NULL	0	NULL	Db MHC class I molecules 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptides were synthesized that correspond to the antigenic sequences from ovalbumin and influenza nucleoprotein believed to be naturally processed and presented by cells with Kb and Db MHC class I molecules , respectively .
	manualset3
122486	1	405005	5	NULL	NULL	0	NULL	Perapion connexum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Perapion connexum ( Schilsky , 1902 ) ( Coleoptera , Apionidae ) in Central Europe , a case of plant expansion chase .
	manualset3
122487	2	405005	5	NULL	NULL	0	NULL	Schilsky , 1902	Citation												NULL		0	NULL	NULL	NULL	NULL	NULL	Perapion connexum ( Schilsky , 1902 ) ( Coleoptera , Apionidae ) in Central Europe , a case of plant expansion chase .
	manualset3
122488	3	405005	5	NULL	NULL	0	NULL	Coleoptera , Apionidae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Perapion connexum ( Schilsky , 1902 ) ( Coleoptera , Apionidae ) in Central Europe , a case of plant expansion chase .
	manualset3
122489	4	405005	5	NULL	NULL	0	NULL	Central Europe	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Perapion connexum ( Schilsky , 1902 ) ( Coleoptera , Apionidae ) in Central Europe , a case of plant expansion chase .
	manualset3
122490	5	405005	5	NULL	NULL	0	NULL	case 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Perapion connexum ( Schilsky , 1902 ) ( Coleoptera , Apionidae ) in Central Europe , a case of plant expansion chase .
	manualset3
122491	6	405005	5	NULL	NULL	NULL	NULL	plant expansion chase	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Perapion connexum ( Schilsky , 1902 ) ( Coleoptera , Apionidae ) in Central Europe , a case of plant expansion chase .
	manualset3
122492	1	405006	5	NULL	NULL	0	NULL	purpose 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Perceived purpose of prescription drugs : the Iowa 65 + Rural Health Study .
	manualset3
122493	2	405006	5	NULL	NULL	0	NULL	prescription drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Perceived purpose of prescription drugs : the Iowa 65 + Rural Health Study .
	manualset3
122494	3	405006	5	NULL	NULL	0	NULL	Iowa 65 + Rural Health Study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Perceived purpose of prescription drugs : the Iowa 65 + Rural Health Study .
	manualset3
122495	1	405007	5	NULL	NULL	0	NULL	Percent body fat	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Percent body fat , serum cholesterol and triglyceride levels were estimated before and after the training program .
	manualset3
122496	2	405007	5	NULL	NULL	0	NULL	serum cholesterol levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Percent body fat , serum cholesterol and triglyceride levels were estimated before and after the training program .
	manualset3
122497	3	405007	5	NULL	NULL	0	NULL	triglyceride levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Percent body fat , serum cholesterol and triglyceride levels were estimated before and after the training program .
	manualset3
122498	4	405007	5	NULL	NULL	0	NULL	training program	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Percent body fat , serum cholesterol and triglyceride levels were estimated before and after the training program .
	manualset3
122499	1	405008	5	NULL	NULL	0	NULL	Percent bone apposition	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Percent bone apposition , trabecular strut width , connectivity index , and cortical porosity measurements were performed at five levels and in four quadrants about the femoral stems .
	manualset3
122500	2	405008	5	NULL	NULL	0	NULL	trabecular strut width	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Percent bone apposition , trabecular strut width , connectivity index , and cortical porosity measurements were performed at five levels and in four quadrants about the femoral stems .
	manualset3
122501	3	405008	5	NULL	NULL	0	NULL	connectivity index	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Percent bone apposition , trabecular strut width , connectivity index , and cortical porosity measurements were performed at five levels and in four quadrants about the femoral stems .
	manualset3
122502	4	405008	5	NULL	NULL	0	NULL	cortical porosity measurements 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Percent bone apposition , trabecular strut width , connectivity index , and cortical porosity measurements were performed at five levels and in four quadrants about the femoral stems .
	manualset3
122503	5	405008	5	NULL	NULL	0	NULL	five levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Percent bone apposition , trabecular strut width , connectivity index , and cortical porosity measurements were performed at five levels and in four quadrants about the femoral stems .
	manualset3
122504	6	405008	5	NULL	NULL	0	NULL	four quadrants	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Percent bone apposition , trabecular strut width , connectivity index , and cortical porosity measurements were performed at five levels and in four quadrants about the femoral stems .
	manualset3
122505	7	405008	5	NULL	NULL	0	NULL	femoral stems	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Percent bone apposition , trabecular strut width , connectivity index , and cortical porosity measurements were performed at five levels and in four quadrants about the femoral stems .
	manualset3
122506	1	405009	5	NULL	NULL	0	NULL	Percent sperm motility 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Percent sperm motility also increased ( p & lt ; 0.05 ) in teratospermic males after swim-up ( 90.0 + / - 1.3 % ) as compared to sperm washing ( 64.2 + / - 3.7 % ) .
	manualset3
122507	2	405009	5	NULL	NULL	0	NULL	 p & lt ; 0.05 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Percent sperm motility also increased ( p & lt ; 0.05 ) in teratospermic males after swim-up ( 90.0 + / - 1.3 % ) as compared to sperm washing ( 64.2 + / - 3.7 % ) .
	manualset3
122508	3	405009	5	NULL	NULL	0	NULL	teratospermic males 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Percent sperm motility also increased ( p & lt ; 0.05 ) in teratospermic males after swim-up ( 90.0 + / - 1.3 % ) as compared to sperm washing ( 64.2 + / - 3.7 % ) .
	manualset3
122509	4	405009	5	NULL	NULL	0	NULL	swim-up	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Percent sperm motility also increased ( p & lt ; 0.05 ) in teratospermic males after swim-up ( 90.0 + / - 1.3 % ) as compared to sperm washing ( 64.2 + / - 3.7 % ) .
	manualset3
122510	5	405009	5	NULL	NULL	0	NULL	 90.0 + / - 1.3 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Percent sperm motility also increased ( p & lt ; 0.05 ) in teratospermic males after swim-up ( 90.0 + / - 1.3 % ) as compared to sperm washing ( 64.2 + / - 3.7 % ) .
	manualset3
122511	6	405009	5	NULL	NULL	0	NULL	sperm washing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Percent sperm motility also increased ( p & lt ; 0.05 ) in teratospermic males after swim-up ( 90.0 + / - 1.3 % ) as compared to sperm washing ( 64.2 + / - 3.7 % ) .
	manualset3
122512	7	405009	5	NULL	NULL	0	NULL	64.2 + / - 3.7 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Percent sperm motility also increased ( p & lt ; 0.05 ) in teratospermic males after swim-up ( 90.0 + / - 1.3 % ) as compared to sperm washing ( 64.2 + / - 3.7 % ) .
	manualset3
122513	1	405010	5	NULL	NULL	NULL	NULL	Percent polarization	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Percent polarization depended on wavelength , where at high sun altitudes maximal percent polarization generally appeared in the UV and red spectral regions .
	manualset3
122514	2	405010	5	NULL	NULL	0	NULL	wavelength 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Percent polarization depended on wavelength , where at high sun altitudes maximal percent polarization generally appeared in the UV and red spectral regions .
	manualset3
122515	3	405010	5	NULL	NULL	0	NULL	high sun altitudes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Percent polarization depended on wavelength , where at high sun altitudes maximal percent polarization generally appeared in the UV and red spectral regions .
	manualset3
122516	4	405010	5	NULL	NULL	NULL	NULL	maximal percent polarization 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Percent polarization depended on wavelength , where at high sun altitudes maximal percent polarization generally appeared in the UV and red spectral regions .
	manualset3
122517	5	405010	5	NULL	NULL	0	NULL	 UV	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Percent polarization depended on wavelength , where at high sun altitudes maximal percent polarization generally appeared in the UV and red spectral regions .
	manualset3
122518	6	405010	5	NULL	NULL	0	NULL	red spectral regions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Percent polarization depended on wavelength , where at high sun altitudes maximal percent polarization generally appeared in the UV and red spectral regions .
	manualset3
122519	1	405011	5	NULL	NULL	NULL	NULL	correlation 	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A good correlation between 50 % inhibitory concentration of hybrid liposomes ( HL ) composed of 90 mol % dimyristoylphosphatidylcholine and 10 mol % polyoxyethylene ( n ) dodecyl ether on the growth of human colon tumor ( WiDr ) cells , and membrane fluidity of HL was obtained .
	manualset3
122520	2	405011	5	NULL	NULL	0	NULL	50 % inhibitory concentration	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A good correlation between 50 % inhibitory concentration of hybrid liposomes ( HL ) composed of 90 mol % dimyristoylphosphatidylcholine and 10 mol % polyoxyethylene ( n ) dodecyl ether on the growth of human colon tumor ( WiDr ) cells , and membrane fluidity of HL was obtained .
	manualset3
122521	3	405011	5	NULL	NULL	0	NULL	hybrid liposomes ( HL )	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A good correlation between 50 % inhibitory concentration of hybrid liposomes ( HL ) composed of 90 mol % dimyristoylphosphatidylcholine and 10 mol % polyoxyethylene ( n ) dodecyl ether on the growth of human colon tumor ( WiDr ) cells , and membrane fluidity of HL was obtained .
	manualset3
122522	4	405011	5	NULL	NULL	0	NULL	90 mol %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A good correlation between 50 % inhibitory concentration of hybrid liposomes ( HL ) composed of 90 mol % dimyristoylphosphatidylcholine and 10 mol % polyoxyethylene ( n ) dodecyl ether on the growth of human colon tumor ( WiDr ) cells , and membrane fluidity of HL was obtained .
	manualset3
122523	5	405011	5	NULL	NULL	0	NULL	dimyristoylphosphatidylcholine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A good correlation between 50 % inhibitory concentration of hybrid liposomes ( HL ) composed of 90 mol % dimyristoylphosphatidylcholine and 10 mol % polyoxyethylene ( n ) dodecyl ether on the growth of human colon tumor ( WiDr ) cells , and membrane fluidity of HL was obtained .
	manualset3
122524	6	405011	5	NULL	NULL	0	NULL	10 mol %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A good correlation between 50 % inhibitory concentration of hybrid liposomes ( HL ) composed of 90 mol % dimyristoylphosphatidylcholine and 10 mol % polyoxyethylene ( n ) dodecyl ether on the growth of human colon tumor ( WiDr ) cells , and membrane fluidity of HL was obtained .
	manualset3
122525	7	405011	5	NULL	NULL	0	NULL	polyoxyethylene ( n ) dodecyl ether	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A good correlation between 50 % inhibitory concentration of hybrid liposomes ( HL ) composed of 90 mol % dimyristoylphosphatidylcholine and 10 mol % polyoxyethylene ( n ) dodecyl ether on the growth of human colon tumor ( WiDr ) cells , and membrane fluidity of HL was obtained .
	manualset3
122526	8	405011	5	NULL	NULL	0	NULL	growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A good correlation between 50 % inhibitory concentration of hybrid liposomes ( HL ) composed of 90 mol % dimyristoylphosphatidylcholine and 10 mol % polyoxyethylene ( n ) dodecyl ether on the growth of human colon tumor ( WiDr ) cells , and membrane fluidity of HL was obtained .
	manualset3
122527	9	405011	5	NULL	NULL	0	NULL	human colon tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A good correlation between 50 % inhibitory concentration of hybrid liposomes ( HL ) composed of 90 mol % dimyristoylphosphatidylcholine and 10 mol % polyoxyethylene ( n ) dodecyl ether on the growth of human colon tumor ( WiDr ) cells , and membrane fluidity of HL was obtained .
	manualset3
122528	10	405011	5	NULL	NULL	0	NULL	( WiDr ) cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A good correlation between 50 % inhibitory concentration of hybrid liposomes ( HL ) composed of 90 mol % dimyristoylphosphatidylcholine and 10 mol % polyoxyethylene ( n ) dodecyl ether on the growth of human colon tumor ( WiDr ) cells , and membrane fluidity of HL was obtained .
	manualset3
122529	11	405011	5	NULL	NULL	0	NULL	membrane fluidity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A good correlation between 50 % inhibitory concentration of hybrid liposomes ( HL ) composed of 90 mol % dimyristoylphosphatidylcholine and 10 mol % polyoxyethylene ( n ) dodecyl ether on the growth of human colon tumor ( WiDr ) cells , and membrane fluidity of HL was obtained .
	manualset3
122530	12	405011	5	NULL	NULL	0	NULL	HL 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A good correlation between 50 % inhibitory concentration of hybrid liposomes ( HL ) composed of 90 mol % dimyristoylphosphatidylcholine and 10 mol % polyoxyethylene ( n ) dodecyl ether on the growth of human colon tumor ( WiDr ) cells , and membrane fluidity of HL was obtained .
	manualset3
122531	1	405012	5	NULL	NULL	0	NULL	Perceptions 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Perceptions of control over work : psychophysiological responses to self-paced and externally-paced tasks in an adult population sample .
	manualset3
122532	2	405012	5	NULL	NULL	0	NULL	control 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Perceptions of control over work : psychophysiological responses to self-paced and externally-paced tasks in an adult population sample .
	manualset3
122533	3	405012	5	NULL	NULL	0	NULL	work 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Perceptions of control over work : psychophysiological responses to self-paced and externally-paced tasks in an adult population sample .
	manualset3
122534	4	405012	5	NULL	NULL	0	NULL	psychophysiological responses	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Perceptions of control over work : psychophysiological responses to self-paced and externally-paced tasks in an adult population sample .
	manualset3
122535	5	405012	5	NULL	NULL	0	NULL	self-paced tasks	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Perceptions of control over work : psychophysiological responses to self-paced and externally-paced tasks in an adult population sample .
	manualset3
122536	6	405012	5	NULL	NULL	0	NULL	externally-paced tasks 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Perceptions of control over work : psychophysiological responses to self-paced and externally-paced tasks in an adult population sample .
	manualset3
122537	7	405012	5	NULL	NULL	0	NULL	adult population sample	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Perceptions of control over work : psychophysiological responses to self-paced and externally-paced tasks in an adult population sample .
	manualset3
122703	1	405013	5	NULL	NULL	0	NULL	Perchlorate 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Perchlorate , iodine supplements , iodized salt and breast milk iodine content .
	manualset3
122704	2	405013	5	NULL	NULL	0	NULL	iodine supplements	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Perchlorate , iodine supplements , iodized salt and breast milk iodine content .
	manualset3
122705	3	405013	5	NULL	NULL	0	NULL	iodized salt	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Perchlorate , iodine supplements , iodized salt and breast milk iodine content .
	manualset3
122706	4	405013	5	NULL	NULL	0	NULL	breast milk iodine content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Perchlorate , iodine supplements , iodized salt and breast milk iodine content .
	manualset3
122707	1	405014	5	NULL	NULL	0	NULL	Percutaneous coronary intervention ( PCI ) 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Percutaneous coronary intervention ( PCI ) for protected left main coronary artery ( PLM ) disease is complex because of patient and lesion factors ; however , limited data exist on the outcomes of drug-eluting stent ( DES ) use for this indication .
	manualset3
122708	2	405014	5	NULL	NULL	0	NULL	protected left main coronary artery ( PLM ) disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Percutaneous coronary intervention ( PCI ) for protected left main coronary artery ( PLM ) disease is complex because of patient and lesion factors ; however , limited data exist on the outcomes of drug-eluting stent ( DES ) use for this indication .
	manualset3
122709	3	405014	5	NULL	NULL	0	NULL	complex 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Percutaneous coronary intervention ( PCI ) for protected left main coronary artery ( PLM ) disease is complex because of patient and lesion factors ; however , limited data exist on the outcomes of drug-eluting stent ( DES ) use for this indication .
	manualset3
122710	4	405014	5	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Percutaneous coronary intervention ( PCI ) for protected left main coronary artery ( PLM ) disease is complex because of patient and lesion factors ; however , limited data exist on the outcomes of drug-eluting stent ( DES ) use for this indication .
	manualset3
122711	5	405014	5	NULL	NULL	0	NULL	lesion factors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Percutaneous coronary intervention ( PCI ) for protected left main coronary artery ( PLM ) disease is complex because of patient and lesion factors ; however , limited data exist on the outcomes of drug-eluting stent ( DES ) use for this indication .
	manualset3
122712	6	405014	5	NULL	NULL	0	NULL	limited data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Percutaneous coronary intervention ( PCI ) for protected left main coronary artery ( PLM ) disease is complex because of patient and lesion factors ; however , limited data exist on the outcomes of drug-eluting stent ( DES ) use for this indication .
	manualset3
122713	7	405014	5	NULL	NULL	0	NULL	outcomes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Percutaneous coronary intervention ( PCI ) for protected left main coronary artery ( PLM ) disease is complex because of patient and lesion factors ; however , limited data exist on the outcomes of drug-eluting stent ( DES ) use for this indication .
	manualset3
122714	8	405014	5	NULL	NULL	0	NULL	drug-eluting stent ( DES )	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Percutaneous coronary intervention ( PCI ) for protected left main coronary artery ( PLM ) disease is complex because of patient and lesion factors ; however , limited data exist on the outcomes of drug-eluting stent ( DES ) use for this indication .
	manualset3
122715	9	405014	5	NULL	NULL	0	NULL	indication 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Percutaneous coronary intervention ( PCI ) for protected left main coronary artery ( PLM ) disease is complex because of patient and lesion factors ; however , limited data exist on the outcomes of drug-eluting stent ( DES ) use for this indication .
	manualset3
122716	1	405015	5	NULL	NULL	0	NULL	Percutaneous drainage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Percutaneous drainage of malignant cysts .
	manualset3
122717	2	405015	5	NULL	NULL	0	NULL	malignant cysts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Percutaneous drainage of malignant cysts .
	manualset3
122718	1	405016	5	NULL	NULL	0	NULL	Percutaneous embolization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Percutaneous embolization of a gastroduodenal artery aneurysm secondary to antrectomy and Roux en Y reconstruction .
	manualset3
122719	2	405016	5	NULL	NULL	0	NULL	gastroduodenal artery aneurysm 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Percutaneous embolization of a gastroduodenal artery aneurysm secondary to antrectomy and Roux en Y reconstruction .
	manualset3
122720	3	405016	5	NULL	NULL	0	NULL	antrectomy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Percutaneous embolization of a gastroduodenal artery aneurysm secondary to antrectomy and Roux en Y reconstruction .
	manualset3
122721	4	405016	5	NULL	NULL	0	NULL	Roux en Y reconstruction	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Percutaneous embolization of a gastroduodenal artery aneurysm secondary to antrectomy and Roux en Y reconstruction .
	manualset3
122722	1	405017	5	NULL	NULL	0	NULL	Percutaneous left ventricular partitioning	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Percutaneous left ventricular partitioning in patients with chronic heart failure and a prior anterior myocardial infarction : Results of the PercutAneous Ventricular RestorAtion in Chronic Heart failUre PaTiEnts Trial .
	manualset3
122723	2	405017	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Percutaneous left ventricular partitioning in patients with chronic heart failure and a prior anterior myocardial infarction : Results of the PercutAneous Ventricular RestorAtion in Chronic Heart failUre PaTiEnts Trial .
	manualset3
122724	3	405017	5	NULL	NULL	0	NULL	chronic heart failure 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Percutaneous left ventricular partitioning in patients with chronic heart failure and a prior anterior myocardial infarction : Results of the PercutAneous Ventricular RestorAtion in Chronic Heart failUre PaTiEnts Trial .
	manualset3
122725	4	405017	5	NULL	NULL	0	NULL	prior anterior myocardial infarction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Percutaneous left ventricular partitioning in patients with chronic heart failure and a prior anterior myocardial infarction : Results of the PercutAneous Ventricular RestorAtion in Chronic Heart failUre PaTiEnts Trial .
	manualset3
122726	5	405017	5	NULL	NULL	0	NULL	Results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Percutaneous left ventricular partitioning in patients with chronic heart failure and a prior anterior myocardial infarction : Results of the PercutAneous Ventricular RestorAtion in Chronic Heart failUre PaTiEnts Trial .
	manualset3
122727	6	405017	5	NULL	NULL	0	NULL	PercutAneous Ventricular RestorAtion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Percutaneous left ventricular partitioning in patients with chronic heart failure and a prior anterior myocardial infarction : Results of the PercutAneous Ventricular RestorAtion in Chronic Heart failUre PaTiEnts Trial .
	manualset3
122728	7	405017	5	NULL	NULL	0	NULL	Chronic Heart failUre PaTiEnts Trial	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Percutaneous left ventricular partitioning in patients with chronic heart failure and a prior anterior myocardial infarction : Results of the PercutAneous Ventricular RestorAtion in Chronic Heart failUre PaTiEnts Trial .
	manualset3
122729	1	405018	5	NULL	NULL	0	NULL	Percutaneous nephrolithotomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Percutaneous nephrolithotomy and its legacy .
	manualset3
122730	2	405018	5	NULL	NULL	0	NULL	legacy 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Percutaneous nephrolithotomy and its legacy .
	manualset3
122731	1	405019	5	NULL	NULL	0	NULL	Perforation of the colon	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Perforation of the colon , which requires surgical intervention more frequently than bleeding , occurs in less than 1 percent of patients undergoing diagnostic colonoscopy and may be seen in up to 3 percent of patients undergoing therapeutic procedures such as polyp removal , dilation of strictures , or laser ablative procedures .
	manualset3
122732	2	405019	5	NULL	NULL	0	NULL	surgical intervention 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Perforation of the colon , which requires surgical intervention more frequently than bleeding , occurs in less than 1 percent of patients undergoing diagnostic colonoscopy and may be seen in up to 3 percent of patients undergoing therapeutic procedures such as polyp removal , dilation of strictures , or laser ablative procedures .
	manualset3
122733	3	405019	5	NULL	NULL	0	NULL	bleeding 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Perforation of the colon , which requires surgical intervention more frequently than bleeding , occurs in less than 1 percent of patients undergoing diagnostic colonoscopy and may be seen in up to 3 percent of patients undergoing therapeutic procedures such as polyp removal , dilation of strictures , or laser ablative procedures .
	manualset3
122734	4	405019	5	NULL	NULL	0	NULL	1 percent	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Perforation of the colon , which requires surgical intervention more frequently than bleeding , occurs in less than 1 percent of patients undergoing diagnostic colonoscopy and may be seen in up to 3 percent of patients undergoing therapeutic procedures such as polyp removal , dilation of strictures , or laser ablative procedures .
	manualset3
122735	5	405019	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Perforation of the colon , which requires surgical intervention more frequently than bleeding , occurs in less than 1 percent of patients undergoing diagnostic colonoscopy and may be seen in up to 3 percent of patients undergoing therapeutic procedures such as polyp removal , dilation of strictures , or laser ablative procedures .
	manualset3
122736	6	405019	5	NULL	NULL	0	NULL	diagnostic colonoscopy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Perforation of the colon , which requires surgical intervention more frequently than bleeding , occurs in less than 1 percent of patients undergoing diagnostic colonoscopy and may be seen in up to 3 percent of patients undergoing therapeutic procedures such as polyp removal , dilation of strictures , or laser ablative procedures .
	manualset3
122737	7	405019	5	NULL	NULL	0	NULL	3 percent	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Perforation of the colon , which requires surgical intervention more frequently than bleeding , occurs in less than 1 percent of patients undergoing diagnostic colonoscopy and may be seen in up to 3 percent of patients undergoing therapeutic procedures such as polyp removal , dilation of strictures , or laser ablative procedures .
	manualset3
122738	8	405019	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Perforation of the colon , which requires surgical intervention more frequently than bleeding , occurs in less than 1 percent of patients undergoing diagnostic colonoscopy and may be seen in up to 3 percent of patients undergoing therapeutic procedures such as polyp removal , dilation of strictures , or laser ablative procedures .
	manualset3
122739	9	405019	5	NULL	NULL	0	NULL	therapeutic procedures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Perforation of the colon , which requires surgical intervention more frequently than bleeding , occurs in less than 1 percent of patients undergoing diagnostic colonoscopy and may be seen in up to 3 percent of patients undergoing therapeutic procedures such as polyp removal , dilation of strictures , or laser ablative procedures .
	manualset3
122740	10	405019	5	NULL	NULL	0	NULL	polyp removal	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Perforation of the colon , which requires surgical intervention more frequently than bleeding , occurs in less than 1 percent of patients undergoing diagnostic colonoscopy and may be seen in up to 3 percent of patients undergoing therapeutic procedures such as polyp removal , dilation of strictures , or laser ablative procedures .
	manualset3
122741	11	405019	5	NULL	NULL	0	NULL	dilation of strictures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Perforation of the colon , which requires surgical intervention more frequently than bleeding , occurs in less than 1 percent of patients undergoing diagnostic colonoscopy and may be seen in up to 3 percent of patients undergoing therapeutic procedures such as polyp removal , dilation of strictures , or laser ablative procedures .
	manualset3
122742	12	405019	5	NULL	NULL	0	NULL	laser ablative procedures 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Perforation of the colon , which requires surgical intervention more frequently than bleeding , occurs in less than 1 percent of patients undergoing diagnostic colonoscopy and may be seen in up to 3 percent of patients undergoing therapeutic procedures such as polyp removal , dilation of strictures , or laser ablative procedures .
	manualset3
122743	1	405020	5	NULL	NULL	0	NULL	Perforator flaps 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Perforator flaps have become standard of care .
	manualset3
122744	2	405020	5	NULL	NULL	0	NULL	standard 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Perforator flaps have become standard of care .
	manualset3
122745	3	405020	5	NULL	NULL	0	NULL	care 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Perforator flaps have become standard of care .
	manualset3
122746	1	405021	5	NULL	NULL	0	NULL	correlation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A good correlation exists between CT , echographic and traditional methodologies findings .
	manualset3
122747	2	405021	5	NULL	NULL	0	NULL	CT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A good correlation exists between CT , echographic and traditional methodologies findings .
	manualset3
122748	3	405021	5	NULL	NULL	0	NULL	echographic findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A good correlation exists between CT , echographic and traditional methodologies findings .
	manualset3
122749	4	405021	5	NULL	NULL	0	NULL	traditional methodologies findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A good correlation exists between CT , echographic and traditional methodologies findings .
	manualset3
122750	1	405022	5	NULL	NULL	0	NULL	Performance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance of an electrocardiogram to evaluate for prolonged QT syndrome should be strongly considered .
	manualset3
122751	2	405022	5	NULL	NULL	0	NULL	electrocardiogram 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance of an electrocardiogram to evaluate for prolonged QT syndrome should be strongly considered .
	manualset3
122753	3	405022	5	NULL	NULL	NULL	NULL	prolonged QT syndrome	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Performance of an electrocardiogram to evaluate for prolonged QT syndrome should be strongly considered .
	manualset3
122754	1	405023	5	NULL	NULL	0	NULL	Performance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance of the block was superior with the Sprotte cannula and the incidence of incomplete blocks was lower ( 1.6 % vs 7.8 % , P = 0.0011 ) .
	manualset3
122755	2	405023	5	NULL	NULL	0	NULL	block 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance of the block was superior with the Sprotte cannula and the incidence of incomplete blocks was lower ( 1.6 % vs 7.8 % , P = 0.0011 ) .
	manualset3
122756	3	405023	5	NULL	NULL	0	NULL	Sprotte cannula	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance of the block was superior with the Sprotte cannula and the incidence of incomplete blocks was lower ( 1.6 % vs 7.8 % , P = 0.0011 ) .
	manualset3
122757	4	405023	5	NULL	NULL	0	NULL	incidence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance of the block was superior with the Sprotte cannula and the incidence of incomplete blocks was lower ( 1.6 % vs 7.8 % , P = 0.0011 ) .
	manualset3
122758	5	405023	5	NULL	NULL	0	NULL	incomplete blocks 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance of the block was superior with the Sprotte cannula and the incidence of incomplete blocks was lower ( 1.6 % vs 7.8 % , P = 0.0011 ) .
	manualset3
122759	6	405023	5	NULL	NULL	0	NULL	1.6 % vs 7.8 % , P = 0.0011	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance of the block was superior with the Sprotte cannula and the incidence of incomplete blocks was lower ( 1.6 % vs 7.8 % , P = 0.0011 ) .
	manualset3
122760	1	405024	5	NULL	NULL	0	NULL	Performance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance of the noninfarcted myocardium therefore seems to have a role in deterioration of left ventricular pump function in acute myocardial infarction
	manualset3
122761	2	405024	5	NULL	NULL	0	NULL	noninfarcted myocardium 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance of the noninfarcted myocardium therefore seems to have a role in deterioration of left ventricular pump function in acute myocardial infarction
	manualset3
122762	3	405024	5	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance of the noninfarcted myocardium therefore seems to have a role in deterioration of left ventricular pump function in acute myocardial infarction
	manualset3
122763	4	405024	5	NULL	NULL	NULL	NULL	deterioration 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Performance of the noninfarcted myocardium therefore seems to have a role in deterioration of left ventricular pump function in acute myocardial infarction
	manualset3
122764	5	405024	5	NULL	NULL	0	NULL	left ventricular pump function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance of the noninfarcted myocardium therefore seems to have a role in deterioration of left ventricular pump function in acute myocardial infarction
	manualset3
122765	6	405024	5	NULL	NULL	0	NULL	acute myocardial infarction 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance of the noninfarcted myocardium therefore seems to have a role in deterioration of left ventricular pump function in acute myocardial infarction
	manualset3
122766	1	405025	5	NULL	NULL	0	NULL	Performance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance of user independent echocardiographic border detection algorithm : comparison with human observer variability .
	manualset3
122767	2	405025	5	NULL	NULL	0	NULL	user independent echocardiographic border detection algorithm	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance of user independent echocardiographic border detection algorithm : comparison with human observer variability .
	manualset3
122768	3	405025	5	NULL	NULL	0	NULL	comparison 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance of user independent echocardiographic border detection algorithm : comparison with human observer variability .
	manualset3
122769	4	405025	5	NULL	NULL	0	NULL	human observer variability	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance of user independent echocardiographic border detection algorithm : comparison with human observer variability .
	manualset3
122770	1	405026	5	NULL	NULL	0	NULL	Performance characteristics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance characteristics of the sutures and needles produced by USS/D & G , which were evaluated in 3407 surgical procedures , included packaging and ease of opening , needle strength and sharpness , tissue drag , knot security , tensile strength , and clinically acceptable and unacceptable determinations .
	manualset3
122771	2	405026	5	NULL	NULL	0	NULL	sutures 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance characteristics of the sutures and needles produced by USS/D & G , which were evaluated in 3407 surgical procedures , included packaging and ease of opening , needle strength and sharpness , tissue drag , knot security , tensile strength , and clinically acceptable and unacceptable determinations .
	manualset3
122772	3	405026	5	NULL	NULL	0	NULL	needles 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance characteristics of the sutures and needles produced by USS/D & G , which were evaluated in 3407 surgical procedures , included packaging and ease of opening , needle strength and sharpness , tissue drag , knot security , tensile strength , and clinically acceptable and unacceptable determinations .
	manualset3
122773	4	405026	5	NULL	NULL	0	NULL	 USS/D & G 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance characteristics of the sutures and needles produced by USS/D & G , which were evaluated in 3407 surgical procedures , included packaging and ease of opening , needle strength and sharpness , tissue drag , knot security , tensile strength , and clinically acceptable and unacceptable determinations .
	manualset3
122774	5	405026	5	NULL	NULL	0	NULL	3407 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance characteristics of the sutures and needles produced by USS/D & G , which were evaluated in 3407 surgical procedures , included packaging and ease of opening , needle strength and sharpness , tissue drag , knot security , tensile strength , and clinically acceptable and unacceptable determinations .
	manualset3
122775	6	405026	5	NULL	NULL	0	NULL	surgical procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance characteristics of the sutures and needles produced by USS/D & G , which were evaluated in 3407 surgical procedures , included packaging and ease of opening , needle strength and sharpness , tissue drag , knot security , tensile strength , and clinically acceptable and unacceptable determinations .
	manualset3
122776	7	405026	5	NULL	NULL	0	NULL	packaging 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance characteristics of the sutures and needles produced by USS/D & G , which were evaluated in 3407 surgical procedures , included packaging and ease of opening , needle strength and sharpness , tissue drag , knot security , tensile strength , and clinically acceptable and unacceptable determinations .
	manualset3
122777	8	405026	5	NULL	NULL	0	NULL	ease 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance characteristics of the sutures and needles produced by USS/D & G , which were evaluated in 3407 surgical procedures , included packaging and ease of opening , needle strength and sharpness , tissue drag , knot security , tensile strength , and clinically acceptable and unacceptable determinations .
	manualset3
122778	9	405026	5	NULL	NULL	0	NULL	opening 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance characteristics of the sutures and needles produced by USS/D & G , which were evaluated in 3407 surgical procedures , included packaging and ease of opening , needle strength and sharpness , tissue drag , knot security , tensile strength , and clinically acceptable and unacceptable determinations .
	manualset3
122779	10	405026	5	NULL	NULL	0	NULL	needle strength	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance characteristics of the sutures and needles produced by USS/D & G , which were evaluated in 3407 surgical procedures , included packaging and ease of opening , needle strength and sharpness , tissue drag , knot security , tensile strength , and clinically acceptable and unacceptable determinations .
	manualset3
122780	11	405026	5	NULL	NULL	0	NULL	sharpness 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance characteristics of the sutures and needles produced by USS/D & G , which were evaluated in 3407 surgical procedures , included packaging and ease of opening , needle strength and sharpness , tissue drag , knot security , tensile strength , and clinically acceptable and unacceptable determinations .
	manualset3
122781	12	405026	5	NULL	NULL	0	NULL	tissue drag	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance characteristics of the sutures and needles produced by USS/D & G , which were evaluated in 3407 surgical procedures , included packaging and ease of opening , needle strength and sharpness , tissue drag , knot security , tensile strength , and clinically acceptable and unacceptable determinations .
	manualset3
122782	13	405026	5	NULL	NULL	0	NULL	knot security	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance characteristics of the sutures and needles produced by USS/D & G , which were evaluated in 3407 surgical procedures , included packaging and ease of opening , needle strength and sharpness , tissue drag , knot security , tensile strength , and clinically acceptable and unacceptable determinations .
	manualset3
122783	14	405026	5	NULL	NULL	0	NULL	tensile strength	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance characteristics of the sutures and needles produced by USS/D & G , which were evaluated in 3407 surgical procedures , included packaging and ease of opening , needle strength and sharpness , tissue drag , knot security , tensile strength , and clinically acceptable and unacceptable determinations .
	manualset3
122784	15	405026	5	NULL	NULL	0	NULL	clinically acceptable and unacceptable determinations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance characteristics of the sutures and needles produced by USS/D & G , which were evaluated in 3407 surgical procedures , included packaging and ease of opening , needle strength and sharpness , tissue drag , knot security , tensile strength , and clinically acceptable and unacceptable determinations .
	manualset3
122785	1	405027	5	NULL	NULL	0	NULL	Performance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance limited by video noise .
	manualset3
122786	2	405027	5	NULL	NULL	0	NULL	video noise	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Performance limited by video noise .
	manualset3
122787	1	405028	5	NULL	NULL	0	NULL	CONDITIONED REFLEXES 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( CONDITIONED REFLEXES IN HIGHER AND LOWER MONKEYS TO COMPLEX EXTERNAL STIMULI ) .
	manualset3
122788	2	405028	5	NULL	NULL	0	NULL	HIGHER MONKEYS	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( CONDITIONED REFLEXES IN HIGHER AND LOWER MONKEYS TO COMPLEX EXTERNAL STIMULI ) .
	manualset3
122789	3	405028	5	NULL	NULL	0	NULL	LOWER MONKEYS	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( CONDITIONED REFLEXES IN HIGHER AND LOWER MONKEYS TO COMPLEX EXTERNAL STIMULI ) .
	manualset3
122790	4	405028	5	NULL	NULL	0	NULL	COMPLEX EXTERNAL STIMULI	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	( CONDITIONED REFLEXES IN HIGHER AND LOWER MONKEYS TO COMPLEX EXTERNAL STIMULI ) .
	manualset3
122791	1	405029	5	NULL	NULL	0	NULL	Perfusion abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion abnormalities in congenital and neoplastic pulmonary disease : comparison of MR perfusion and multislice CT imaging .
	manualset3
122792	2	405029	5	NULL	NULL	0	NULL	congenital pulmonary disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion abnormalities in congenital and neoplastic pulmonary disease : comparison of MR perfusion and multislice CT imaging .
	manualset3
122793	3	405029	5	NULL	NULL	0	NULL	neoplastic pulmonary disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion abnormalities in congenital and neoplastic pulmonary disease : comparison of MR perfusion and multislice CT imaging .
	manualset3
122794	4	405029	5	NULL	NULL	0	NULL	comparison 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion abnormalities in congenital and neoplastic pulmonary disease : comparison of MR perfusion and multislice CT imaging .
	manualset3
122795	5	405029	5	NULL	NULL	0	NULL	MR perfusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion abnormalities in congenital and neoplastic pulmonary disease : comparison of MR perfusion and multislice CT imaging .
	manualset3
122796	6	405029	5	NULL	NULL	0	NULL	multislice CT imaging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion abnormalities in congenital and neoplastic pulmonary disease : comparison of MR perfusion and multislice CT imaging .
	manualset3
122797	1	405030	5	NULL	NULL	0	NULL	Perfusion of lungs 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion of lungs with Krebs solution containing dipyridamole ( 1-100 microM ) or adenine ( 10 microM ) increased the rate of radioactive efflux , decreased uptake of radioactivity by lung and decreased metabolites of adenosine ( inosine and hypoxanthine ) in the effluent .
	manualset3
122798	2	405030	5	NULL	NULL	0	NULL	Krebs solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion of lungs with Krebs solution containing dipyridamole ( 1-100 microM ) or adenine ( 10 microM ) increased the rate of radioactive efflux , decreased uptake of radioactivity by lung and decreased metabolites of adenosine ( inosine and hypoxanthine ) in the effluent .
	manualset3
122799	3	405030	5	NULL	NULL	0	NULL	dipyridamole 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion of lungs with Krebs solution containing dipyridamole ( 1-100 microM ) or adenine ( 10 microM ) increased the rate of radioactive efflux , decreased uptake of radioactivity by lung and decreased metabolites of adenosine ( inosine and hypoxanthine ) in the effluent .
	manualset3
122800	4	405030	5	NULL	NULL	0	NULL	1-100 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion of lungs with Krebs solution containing dipyridamole ( 1-100 microM ) or adenine ( 10 microM ) increased the rate of radioactive efflux , decreased uptake of radioactivity by lung and decreased metabolites of adenosine ( inosine and hypoxanthine ) in the effluent .
	manualset3
122808	5	405030	5	NULL	NULL	0	NULL	adenine 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion of lungs with Krebs solution containing dipyridamole ( 1-100 microM ) or adenine ( 10 microM ) increased the rate of radioactive efflux , decreased uptake of radioactivity by lung and decreased metabolites of adenosine ( inosine and hypoxanthine ) in the effluent .
	manualset3
122809	6	405030	5	NULL	NULL	0	NULL	10 microM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion of lungs with Krebs solution containing dipyridamole ( 1-100 microM ) or adenine ( 10 microM ) increased the rate of radioactive efflux , decreased uptake of radioactivity by lung and decreased metabolites of adenosine ( inosine and hypoxanthine ) in the effluent .
	manualset3
122810	7	405030	5	NULL	NULL	0	NULL	rate 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion of lungs with Krebs solution containing dipyridamole ( 1-100 microM ) or adenine ( 10 microM ) increased the rate of radioactive efflux , decreased uptake of radioactivity by lung and decreased metabolites of adenosine ( inosine and hypoxanthine ) in the effluent .
	manualset3
122811	8	405030	5	NULL	NULL	NULL	NULL	radioactive efflux	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Perfusion of lungs with Krebs solution containing dipyridamole ( 1-100 microM ) or adenine ( 10 microM ) increased the rate of radioactive efflux , decreased uptake of radioactivity by lung and decreased metabolites of adenosine ( inosine and hypoxanthine ) in the effluent .
	manualset3
122812	9	405030	5	NULL	NULL	0	NULL	decreased uptake 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion of lungs with Krebs solution containing dipyridamole ( 1-100 microM ) or adenine ( 10 microM ) increased the rate of radioactive efflux , decreased uptake of radioactivity by lung and decreased metabolites of adenosine ( inosine and hypoxanthine ) in the effluent .
	manualset3
122813	10	405030	5	NULL	NULL	0	NULL	radioactivity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion of lungs with Krebs solution containing dipyridamole ( 1-100 microM ) or adenine ( 10 microM ) increased the rate of radioactive efflux , decreased uptake of radioactivity by lung and decreased metabolites of adenosine ( inosine and hypoxanthine ) in the effluent .
	manualset3
122814	11	405030	5	NULL	NULL	0	NULL	lung 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion of lungs with Krebs solution containing dipyridamole ( 1-100 microM ) or adenine ( 10 microM ) increased the rate of radioactive efflux , decreased uptake of radioactivity by lung and decreased metabolites of adenosine ( inosine and hypoxanthine ) in the effluent .
	manualset3
122815	12	405030	5	NULL	NULL	NULL	NULL	 metabolites of adenosine ( inosine and hypoxanthine )	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Perfusion of lungs with Krebs solution containing dipyridamole ( 1-100 microM ) or adenine ( 10 microM ) increased the rate of radioactive efflux , decreased uptake of radioactivity by lung and decreased metabolites of adenosine ( inosine and hypoxanthine ) in the effluent .
	manualset3
122816	13	405030	5	NULL	NULL	0	NULL	effluent 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion of lungs with Krebs solution containing dipyridamole ( 1-100 microM ) or adenine ( 10 microM ) increased the rate of radioactive efflux , decreased uptake of radioactivity by lung and decreased metabolites of adenosine ( inosine and hypoxanthine ) in the effluent .
	manualset3
122827	1	405031	5	NULL	NULL	NULL	NULL	Perfusion 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Perfusion of two isolated brains from immature male rhesus monkeys with ( ( 3 ) H ) androstenedione resulted in the identification of free and conjugated ( ( 3 ) H ) estrone and free ( ( 3 ) H ) estradiol from the perfusates .
	manualset3
122829	2	405031	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion of two isolated brains from immature male rhesus monkeys with ( ( 3 ) H ) androstenedione resulted in the identification of free and conjugated ( ( 3 ) H ) estrone and free ( ( 3 ) H ) estradiol from the perfusates .
	manualset3
122831	3	405031	5	NULL	NULL	0	NULL	isolated brains 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion of two isolated brains from immature male rhesus monkeys with ( ( 3 ) H ) androstenedione resulted in the identification of free and conjugated ( ( 3 ) H ) estrone and free ( ( 3 ) H ) estradiol from the perfusates .
	manualset3
122832	4	405031	5	NULL	NULL	0	NULL	immature male rhesus monkeys	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion of two isolated brains from immature male rhesus monkeys with ( ( 3 ) H ) androstenedione resulted in the identification of free and conjugated ( ( 3 ) H ) estrone and free ( ( 3 ) H ) estradiol from the perfusates .
	manualset3
122833	5	405031	5	NULL	NULL	0	NULL	 ( ( 3 ) H ) androstenedione	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion of two isolated brains from immature male rhesus monkeys with ( ( 3 ) H ) androstenedione resulted in the identification of free and conjugated ( ( 3 ) H ) estrone and free ( ( 3 ) H ) estradiol from the perfusates .
	manualset3
122834	6	405031	5	NULL	NULL	0	NULL	identification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion of two isolated brains from immature male rhesus monkeys with ( ( 3 ) H ) androstenedione resulted in the identification of free and conjugated ( ( 3 ) H ) estrone and free ( ( 3 ) H ) estradiol from the perfusates .
	manualset3
122838	7	405031	5	NULL	NULL	0	NULL	free ( ( 3 ) H ) estrone 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion of two isolated brains from immature male rhesus monkeys with ( ( 3 ) H ) androstenedione resulted in the identification of free and conjugated ( ( 3 ) H ) estrone and free ( ( 3 ) H ) estradiol from the perfusates .
	manualset3
122840	8	405031	5	NULL	NULL	0	NULL	conjugated ( ( 3 ) H ) estrone 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion of two isolated brains from immature male rhesus monkeys with ( ( 3 ) H ) androstenedione resulted in the identification of free and conjugated ( ( 3 ) H ) estrone and free ( ( 3 ) H ) estradiol from the perfusates .
	manualset3
122842	9	405031	5	NULL	NULL	0	NULL	free ( ( 3 ) H ) estradiol 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion of two isolated brains from immature male rhesus monkeys with ( ( 3 ) H ) androstenedione resulted in the identification of free and conjugated ( ( 3 ) H ) estrone and free ( ( 3 ) H ) estradiol from the perfusates .
	manualset3
122845	10	405031	5	NULL	NULL	0	NULL	perfusates 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion of two isolated brains from immature male rhesus monkeys with ( ( 3 ) H ) androstenedione resulted in the identification of free and conjugated ( ( 3 ) H ) estrone and free ( ( 3 ) H ) estradiol from the perfusates .
	manualset3
122854	1	405032	5	NULL	NULL	0	NULL	Perfusion studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion studies with the intact liver have the fundamental advantage that the structural and functional organization of the liver is preserved ; however , the experimental system is more complex in view of subcellular and intercellular compartmentation and the recently demonstrated metabolic interactions of different cell populations at the acinar level .
	manualset3
122855	2	405032	5	NULL	NULL	0	NULL	intact liver 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion studies with the intact liver have the fundamental advantage that the structural and functional organization of the liver is preserved ; however , the experimental system is more complex in view of subcellular and intercellular compartmentation and the recently demonstrated metabolic interactions of different cell populations at the acinar level .
	manualset3
122856	3	405032	5	NULL	NULL	0	NULL	fundamental advantage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion studies with the intact liver have the fundamental advantage that the structural and functional organization of the liver is preserved ; however , the experimental system is more complex in view of subcellular and intercellular compartmentation and the recently demonstrated metabolic interactions of different cell populations at the acinar level .
	manualset3
122857	4	405032	5	NULL	NULL	0	NULL	structural organization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion studies with the intact liver have the fundamental advantage that the structural and functional organization of the liver is preserved ; however , the experimental system is more complex in view of subcellular and intercellular compartmentation and the recently demonstrated metabolic interactions of different cell populations at the acinar level .
	manualset3
122858	5	405032	5	NULL	NULL	0	NULL	functional organization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion studies with the intact liver have the fundamental advantage that the structural and functional organization of the liver is preserved ; however , the experimental system is more complex in view of subcellular and intercellular compartmentation and the recently demonstrated metabolic interactions of different cell populations at the acinar level .
	manualset3
122860	6	405032	5	NULL	NULL	0	NULL	liver 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion studies with the intact liver have the fundamental advantage that the structural and functional organization of the liver is preserved ; however , the experimental system is more complex in view of subcellular and intercellular compartmentation and the recently demonstrated metabolic interactions of different cell populations at the acinar level .
	manualset3
122862	7	405032	5	NULL	NULL	0	NULL	experimental system	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion studies with the intact liver have the fundamental advantage that the structural and functional organization of the liver is preserved ; however , the experimental system is more complex in view of subcellular and intercellular compartmentation and the recently demonstrated metabolic interactions of different cell populations at the acinar level .
	manualset3
122863	8	405032	5	NULL	NULL	0	NULL	complex 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion studies with the intact liver have the fundamental advantage that the structural and functional organization of the liver is preserved ; however , the experimental system is more complex in view of subcellular and intercellular compartmentation and the recently demonstrated metabolic interactions of different cell populations at the acinar level .
	manualset3
122864	9	405032	5	NULL	NULL	0	NULL	view 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion studies with the intact liver have the fundamental advantage that the structural and functional organization of the liver is preserved ; however , the experimental system is more complex in view of subcellular and intercellular compartmentation and the recently demonstrated metabolic interactions of different cell populations at the acinar level .
	manualset3
122867	10	405032	5	NULL	NULL	0	NULL	subcellular compartmentation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion studies with the intact liver have the fundamental advantage that the structural and functional organization of the liver is preserved ; however , the experimental system is more complex in view of subcellular and intercellular compartmentation and the recently demonstrated metabolic interactions of different cell populations at the acinar level .
	manualset3
122868	11	405032	5	NULL	NULL	0	NULL	intercellular compartmentation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion studies with the intact liver have the fundamental advantage that the structural and functional organization of the liver is preserved ; however , the experimental system is more complex in view of subcellular and intercellular compartmentation and the recently demonstrated metabolic interactions of different cell populations at the acinar level .
	manualset3
122869	12	405032	5	NULL	NULL	0	NULL	metabolic interactions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion studies with the intact liver have the fundamental advantage that the structural and functional organization of the liver is preserved ; however , the experimental system is more complex in view of subcellular and intercellular compartmentation and the recently demonstrated metabolic interactions of different cell populations at the acinar level .
	manualset3
122871	13	405032	5	NULL	NULL	0	NULL	different cell populations	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion studies with the intact liver have the fundamental advantage that the structural and functional organization of the liver is preserved ; however , the experimental system is more complex in view of subcellular and intercellular compartmentation and the recently demonstrated metabolic interactions of different cell populations at the acinar level .
	manualset3
122874	14	405032	5	NULL	NULL	0	NULL	acinar level	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion studies with the intact liver have the fundamental advantage that the structural and functional organization of the liver is preserved ; however , the experimental system is more complex in view of subcellular and intercellular compartmentation and the recently demonstrated metabolic interactions of different cell populations at the acinar level .
	manualset3
122877	1	405033	5	NULL	NULL	0	NULL	Perfusion 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion with post-ischemic hepatic effluent caused a transient 15-min increase in left ventricular contraction and coronary flow ( p & lt ; 0.05 ) , followed by a decrease in cardiac function at one hour .
	manualset3
122879	2	405033	5	NULL	NULL	0	NULL	post-ischemic hepatic effluent 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion with post-ischemic hepatic effluent caused a transient 15-min increase in left ventricular contraction and coronary flow ( p & lt ; 0.05 ) , followed by a decrease in cardiac function at one hour .
	manualset3
122882	3	405033	5	NULL	NULL	0	NULL	transient 15-min increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion with post-ischemic hepatic effluent caused a transient 15-min increase in left ventricular contraction and coronary flow ( p & lt ; 0.05 ) , followed by a decrease in cardiac function at one hour .
	manualset3
122884	4	405033	5	NULL	NULL	0	NULL	left ventricular contraction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion with post-ischemic hepatic effluent caused a transient 15-min increase in left ventricular contraction and coronary flow ( p & lt ; 0.05 ) , followed by a decrease in cardiac function at one hour .
	manualset3
122886	5	405033	5	NULL	NULL	0	NULL	coronary flow	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion with post-ischemic hepatic effluent caused a transient 15-min increase in left ventricular contraction and coronary flow ( p & lt ; 0.05 ) , followed by a decrease in cardiac function at one hour .
	manualset3
122887	6	405033	5	NULL	NULL	0	NULL	p & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion with post-ischemic hepatic effluent caused a transient 15-min increase in left ventricular contraction and coronary flow ( p & lt ; 0.05 ) , followed by a decrease in cardiac function at one hour .
	manualset3
122888	7	405033	5	NULL	NULL	0	NULL	decrease 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion with post-ischemic hepatic effluent caused a transient 15-min increase in left ventricular contraction and coronary flow ( p & lt ; 0.05 ) , followed by a decrease in cardiac function at one hour .
	manualset3
122889	8	405033	5	NULL	NULL	0	NULL	cardiac function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion with post-ischemic hepatic effluent caused a transient 15-min increase in left ventricular contraction and coronary flow ( p & lt ; 0.05 ) , followed by a decrease in cardiac function at one hour .
	manualset3
122890	9	405033	5	NULL	NULL	0	NULL	one hour	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Perfusion with post-ischemic hepatic effluent caused a transient 15-min increase in left ventricular contraction and coronary flow ( p & lt ; 0.05 ) , followed by a decrease in cardiac function at one hour .
	manualset3
122891	1	405034	5	NULL	NULL	0	NULL	variablity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Perhaps , this variablity also contribute to the susceptibility for granulocyte vasculitis and requires future studies .
	manualset3
122892	2	405034	5	NULL	NULL	0	NULL	susceptibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Perhaps , this variablity also contribute to the susceptibility for granulocyte vasculitis and requires future studies .
	manualset3
122893	3	405034	5	NULL	NULL	0	NULL	granulocyte vasculitis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Perhaps , this variablity also contribute to the susceptibility for granulocyte vasculitis and requires future studies .
	manualset3
122894	4	405034	5	NULL	NULL	0	NULL	future studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Perhaps , this variablity also contribute to the susceptibility for granulocyte vasculitis and requires future studies .
	manualset3
122895	1	405035	5	NULL	NULL	0	NULL	 over expression	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Perhaps over expression of GALC activity may be detrimental to oligodendrocytes .
	manualset3
122896	2	405035	5	NULL	NULL	0	NULL	GALC activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Perhaps over expression of GALC activity may be detrimental to oligodendrocytes .
	manualset3
122897	3	405035	5	NULL	NULL	0	NULL	oligodendrocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Perhaps over expression of GALC activity may be detrimental to oligodendrocytes .
	manualset3
122898	1	405036	5	NULL	NULL	0	NULL	challenging obstacle 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Perhaps the most challenging obstacle to rigor in these studies lies in determining which events of condom-protected sex occurred before infection as opposed to after infection when , in fact , infection occurs .
	manualset3
122899	2	405036	5	NULL	NULL	0	NULL	rigor 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Perhaps the most challenging obstacle to rigor in these studies lies in determining which events of condom-protected sex occurred before infection as opposed to after infection when , in fact , infection occurs .
	manualset3
122901	3	405036	5	NULL	NULL	0	NULL	events 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Perhaps the most challenging obstacle to rigor in these studies lies in determining which events of condom-protected sex occurred before infection as opposed to after infection when , in fact , infection occurs .
	manualset3
122904	4	405036	5	NULL	NULL	0	NULL	condom-protected sex	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Perhaps the most challenging obstacle to rigor in these studies lies in determining which events of condom-protected sex occurred before infection as opposed to after infection when , in fact , infection occurs .
	manualset3
122905	5	405036	5	NULL	NULL	0	NULL	infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Perhaps the most challenging obstacle to rigor in these studies lies in determining which events of condom-protected sex occurred before infection as opposed to after infection when , in fact , infection occurs .
	manualset3
122906	6	405036	5	NULL	NULL	0	NULL	infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Perhaps the most challenging obstacle to rigor in these studies lies in determining which events of condom-protected sex occurred before infection as opposed to after infection when , in fact , infection occurs .
	manualset3
122907	7	405036	5	NULL	NULL	0	NULL	infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Perhaps the most challenging obstacle to rigor in these studies lies in determining which events of condom-protected sex occurred before infection as opposed to after infection when , in fact , infection occurs .
	manualset3
128808	8	405036	5	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Perhaps the most challenging obstacle to rigor in these studies lies in determining which events of condom-protected sex occurred before infection as opposed to after infection when , in fact , infection occurs .
	manualset3
122918	1	405037	5	NULL	NULL	0	NULL	Perhydroderivatives of polyene antibiotics	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Perhydroderivatives of polyene antibiotics have a much lower activity against eukaryotic cells than the polyene antibiotics itself .
	manualset3
122919	2	405037	5	NULL	NULL	0	NULL	lower activity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Perhydroderivatives of polyene antibiotics have a much lower activity against eukaryotic cells than the polyene antibiotics itself .
	manualset3
122920	3	405037	5	NULL	NULL	0	NULL	eukaryotic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Perhydroderivatives of polyene antibiotics have a much lower activity against eukaryotic cells than the polyene antibiotics itself .
	manualset3
122925	4	405037	5	NULL	NULL	0	NULL	polyene antibiotics	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Perhydroderivatives of polyene antibiotics have a much lower activity against eukaryotic cells than the polyene antibiotics itself .
	manualset3
122928	1	405038	5	NULL	NULL	0	NULL	Periodic cdc25C transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Periodic cdc25C transcription is mediated by a novel cell cycle-regulated repressor element ( CDE ) .
	manualset3
122929	2	405038	5	NULL	NULL	0	NULL	novel cell cycle-regulated repressor element ( CDE )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Periodic cdc25C transcription is mediated by a novel cell cycle-regulated repressor element ( CDE ) .
	manualset3
122930	1	405039	5	NULL	NULL	0	NULL	relative correspondence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A good relative correspondence between theoretical and measured CCSs was obtained allowing the identification of the exact position of the biotransformation .
	manualset3
122965	2	405039	5	NULL	NULL	0	NULL	theoretical CCSs	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A good relative correspondence between theoretical and measured CCSs was obtained allowing the identification of the exact position of the biotransformation .
	manualset3
122966	3	405039	5	NULL	NULL	0	NULL	measured CCSs 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A good relative correspondence between theoretical and measured CCSs was obtained allowing the identification of the exact position of the biotransformation .
	manualset3
122968	4	405039	5	NULL	NULL	0	NULL	identification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A good relative correspondence between theoretical and measured CCSs was obtained allowing the identification of the exact position of the biotransformation .
	manualset3
122970	5	405039	5	NULL	NULL	0	NULL	exact position	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A good relative correspondence between theoretical and measured CCSs was obtained allowing the identification of the exact position of the biotransformation .
	manualset3
122973	6	405039	5	NULL	NULL	0	NULL	biotransformation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A good relative correspondence between theoretical and measured CCSs was obtained allowing the identification of the exact position of the biotransformation .
	manualset3
122975	1	405040	5	NULL	NULL	0	NULL	Periodontitis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Periodontitis is characterized by loss of tooth-supporting structures and alveolar bone resorption .
	manualset3
122977	2	405040	5	NULL	NULL	0	NULL	loss 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Periodontitis is characterized by loss of tooth-supporting structures and alveolar bone resorption .
	manualset3
122978	3	405040	5	NULL	NULL	0	NULL	tooth-supporting structures	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Periodontitis is characterized by loss of tooth-supporting structures and alveolar bone resorption .
	manualset3
122980	4	405040	5	NULL	NULL	0	NULL	alveolar bone resorption	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Periodontitis is characterized by loss of tooth-supporting structures and alveolar bone resorption .
	manualset3
122983	1	405041	5	NULL	NULL	0	NULL	Peripheral Nervous System Function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral Nervous System Function and Organophosphate Pesticide Use among Licensed Pesticide Applicators in the Agricultural Health Study .
	manualset3
122991	2	405041	5	NULL	NULL	0	NULL	Organophosphate Pesticide Use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral Nervous System Function and Organophosphate Pesticide Use among Licensed Pesticide Applicators in the Agricultural Health Study .
	manualset3
123089	3	405041	5	NULL	NULL	0	NULL	Licensed Pesticide Applicators	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral Nervous System Function and Organophosphate Pesticide Use among Licensed Pesticide Applicators in the Agricultural Health Study .
	manualset3
123090	4	405041	5	NULL	NULL	0	NULL	Agricultural Health Study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral Nervous System Function and Organophosphate Pesticide Use among Licensed Pesticide Applicators in the Agricultural Health Study .
	manualset3
123091	1	405042	5	NULL	NULL	NULL	NULL	Peripheral administration	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Peripheral administration of RU 38486 did not affect fear-related levels of freezing immediately following a footshock or in a long-term memory test 24 h later .
	manualset3
123092	2	405042	5	NULL	NULL	0	NULL	RU 38486	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral administration of RU 38486 did not affect fear-related levels of freezing immediately following a footshock or in a long-term memory test 24 h later .
	manualset3
123093	3	405042	5	NULL	NULL	0	NULL	affect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral administration of RU 38486 did not affect fear-related levels of freezing immediately following a footshock or in a long-term memory test 24 h later .
	manualset3
123094	4	405042	5	NULL	NULL	0	NULL	fear-related levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral administration of RU 38486 did not affect fear-related levels of freezing immediately following a footshock or in a long-term memory test 24 h later .
	manualset3
123095	5	405042	5	NULL	NULL	0	NULL	footshock 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral administration of RU 38486 did not affect fear-related levels of freezing immediately following a footshock or in a long-term memory test 24 h later .
	manualset3
123096	6	405042	5	NULL	NULL	0	NULL	long-term memory test	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral administration of RU 38486 did not affect fear-related levels of freezing immediately following a footshock or in a long-term memory test 24 h later .
	manualset3
123097	7	405042	5	NULL	NULL	0	NULL	24 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral administration of RU 38486 did not affect fear-related levels of freezing immediately following a footshock or in a long-term memory test 24 h later .
	manualset3
123098	1	405043	5	NULL	NULL	0	NULL	Peripheral blood progenitor cell cycle kinetics	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral blood progenitor cell cycle kinetics following priming with pIXY321 in patients treated with the `` ICE '' regimen .
	manualset3
123099	2	405043	5	NULL	NULL	0	NULL	priming 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral blood progenitor cell cycle kinetics following priming with pIXY321 in patients treated with the `` ICE '' regimen .
	manualset3
123100	3	405043	5	NULL	NULL	0	NULL	pIXY321 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral blood progenitor cell cycle kinetics following priming with pIXY321 in patients treated with the `` ICE '' regimen .
	manualset3
123101	4	405043	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral blood progenitor cell cycle kinetics following priming with pIXY321 in patients treated with the `` ICE '' regimen .
	manualset3
123102	5	405043	5	NULL	NULL	NULL	NULL	 `` ICE '' regimen	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Peripheral blood progenitor cell cycle kinetics following priming with pIXY321 in patients treated with the `` ICE '' regimen .
	manualset3
123103	1	405044	5	NULL	NULL	0	NULL	Peripheral neuropathy 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral neuropathy and cold agglutinin hemolytic anemia are the most common reported and occur in 5-10 % of patients .
	manualset3
123104	2	405044	5	NULL	NULL	0	NULL	cold agglutinin hemolytic anemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral neuropathy and cold agglutinin hemolytic anemia are the most common reported and occur in 5-10 % of patients .
	manualset3
123105	3	405044	5	NULL	NULL	0	NULL	 5-10 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral neuropathy and cold agglutinin hemolytic anemia are the most common reported and occur in 5-10 % of patients .
	manualset3
123106	4	405044	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral neuropathy and cold agglutinin hemolytic anemia are the most common reported and occur in 5-10 % of patients .
	manualset3
123107	1	405045	5	NULL	NULL	0	NULL	Peripheral vasodilation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral vasodilation : methods of evaluation and the correlation with clinical practice .
	manualset3
123108	2	405045	5	NULL	NULL	0	NULL	methods 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral vasodilation : methods of evaluation and the correlation with clinical practice .
	manualset3
123109	3	405045	5	NULL	NULL	0	NULL	evaluation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral vasodilation : methods of evaluation and the correlation with clinical practice .
	manualset3
123110	4	405045	5	NULL	NULL	0	NULL	correlation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral vasodilation : methods of evaluation and the correlation with clinical practice .
	manualset3
123111	5	405045	5	NULL	NULL	0	NULL	clinical practice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral vasodilation : methods of evaluation and the correlation with clinical practice .
	manualset3
123116	1	405046	5	NULL	NULL	0	NULL	gradient 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A gradient of prognostic strength of diagnostic measures was EEG phase greater than EEG coherence greater than GCS-T greater than CT-scan greater than EEG relative power .
	manualset3
123117	2	405046	5	NULL	NULL	0	NULL	prognostic strength	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A gradient of prognostic strength of diagnostic measures was EEG phase greater than EEG coherence greater than GCS-T greater than CT-scan greater than EEG relative power .
	manualset3
123122	3	405046	5	NULL	NULL	0	NULL	diagnostic measures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A gradient of prognostic strength of diagnostic measures was EEG phase greater than EEG coherence greater than GCS-T greater than CT-scan greater than EEG relative power .
	manualset3
123130	4	405046	5	NULL	NULL	0	NULL	EEG phase 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A gradient of prognostic strength of diagnostic measures was EEG phase greater than EEG coherence greater than GCS-T greater than CT-scan greater than EEG relative power .
	manualset3
123131	5	405046	5	NULL	NULL	0	NULL	EEG coherence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A gradient of prognostic strength of diagnostic measures was EEG phase greater than EEG coherence greater than GCS-T greater than CT-scan greater than EEG relative power .
	manualset3
123133	6	405046	5	NULL	NULL	0	NULL	GCS-T 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A gradient of prognostic strength of diagnostic measures was EEG phase greater than EEG coherence greater than GCS-T greater than CT-scan greater than EEG relative power .
	manualset3
123134	7	405046	5	NULL	NULL	0	NULL	CT-scan	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A gradient of prognostic strength of diagnostic measures was EEG phase greater than EEG coherence greater than GCS-T greater than CT-scan greater than EEG relative power .
	manualset3
123135	8	405046	5	NULL	NULL	0	NULL	EEG relative power	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A gradient of prognostic strength of diagnostic measures was EEG phase greater than EEG coherence greater than GCS-T greater than CT-scan greater than EEG relative power .
	manualset3
123143	1	405047	5	NULL	NULL	0	NULL	Peripheral vision	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral vision and optokinetic nystagmus in children with unilateral congenital cataract .
	manualset3
123148	2	405047	5	NULL	NULL	0	NULL	optokinetic nystagmus	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral vision and optokinetic nystagmus in children with unilateral congenital cataract .
	manualset3
123150	3	405047	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral vision and optokinetic nystagmus in children with unilateral congenital cataract .
	manualset3
123152	4	405047	5	NULL	NULL	0	NULL	unilateral congenital cataract 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral vision and optokinetic nystagmus in children with unilateral congenital cataract .
	manualset3
123153	1	405048	5	NULL	NULL	0	NULL	Periplasmic expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Periplasmic expression of part of the major rotavirus capsid protein VP7 containing all the three antigenic regions in Escherichia coli .
	manualset3
123154	2	405048	5	NULL	NULL	0	NULL	part of the major rotavirus capsid protein VP7 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Periplasmic expression of part of the major rotavirus capsid protein VP7 containing all the three antigenic regions in Escherichia coli .
	manualset3
123155	3	405048	5	NULL	NULL	0	NULL	three 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Periplasmic expression of part of the major rotavirus capsid protein VP7 containing all the three antigenic regions in Escherichia coli .
	manualset3
123156	4	405048	5	NULL	NULL	0	NULL	antigenic regions	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Periplasmic expression of part of the major rotavirus capsid protein VP7 containing all the three antigenic regions in Escherichia coli .
	manualset3
123157	5	405048	5	NULL	NULL	0	NULL	Escherichia coli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Periplasmic expression of part of the major rotavirus capsid protein VP7 containing all the three antigenic regions in Escherichia coli .
	manualset3
123158	1	405049	5	NULL	NULL	0	NULL	Peripubertal anxiety profile	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripubertal anxiety profile can predict predisposition to spatial memory impairments following chronic stress .
	manualset3
123172	2	405049	5	NULL	NULL	0	NULL	predisposition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripubertal anxiety profile can predict predisposition to spatial memory impairments following chronic stress .
	manualset3
123173	3	405049	5	NULL	NULL	0	NULL	spatial memory impairments 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripubertal anxiety profile can predict predisposition to spatial memory impairments following chronic stress .
	manualset3
123176	4	405049	5	NULL	NULL	0	NULL	chronic stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripubertal anxiety profile can predict predisposition to spatial memory impairments following chronic stress .
	manualset3
123186	1	405050	5	NULL	NULL	0	NULL	Perirenal hematoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Perirenal hematoma in association with renal infarction in sickle-cell trait .
	manualset3
123187	2	405050	5	NULL	NULL	0	NULL	association 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Perirenal hematoma in association with renal infarction in sickle-cell trait .
	manualset3
123403	3	405050	5	NULL	NULL	0	NULL	renal infarction	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Perirenal hematoma in association with renal infarction in sickle-cell trait .
	manualset3
123404	4	405050	5	NULL	NULL	0	NULL	sickle-cell trait	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Perirenal hematoma in association with renal infarction in sickle-cell trait .
	manualset3
123405	1	405051	5	NULL	NULL	NULL	NULL	Peritoneal exudate cells isolated on day 14 ( PEC14 )	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Peritoneal exudate cells isolated on day 14 ( PEC14 ) from mice cured of SL2 tumor were highly effective in Winn Assays .
	manualset3
123406	2	405051	5	NULL	NULL	0	NULL	mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Peritoneal exudate cells isolated on day 14 ( PEC14 ) from mice cured of SL2 tumor were highly effective in Winn Assays .
	manualset3
123407	3	405051	5	NULL	NULL	0	NULL	 SL2 tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Peritoneal exudate cells isolated on day 14 ( PEC14 ) from mice cured of SL2 tumor were highly effective in Winn Assays .
	manualset3
123408	4	405051	5	NULL	NULL	0	NULL	Winn Assays 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Peritoneal exudate cells isolated on day 14 ( PEC14 ) from mice cured of SL2 tumor were highly effective in Winn Assays .
	manualset3
123409	1	405052	5	NULL	NULL	0	NULL	Permeability and conductivity ratios 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Permeability and conductivity ratios were distinct for cells dialyzed with Na ( + ) - or K ( + ) - based internal solution , and application of external glutamate altered anion permeability ratios and the concentration dependence of the anion influx .
	manualset3
123410	2	405052	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Permeability and conductivity ratios were distinct for cells dialyzed with Na ( + ) - or K ( + ) - based internal solution , and application of external glutamate altered anion permeability ratios and the concentration dependence of the anion influx .
	manualset3
123411	3	405052	5	NULL	NULL	0	NULL	 Na ( + )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Permeability and conductivity ratios were distinct for cells dialyzed with Na ( + ) - or K ( + ) - based internal solution , and application of external glutamate altered anion permeability ratios and the concentration dependence of the anion influx .
	manualset3
123412	4	405052	5	NULL	NULL	0	NULL	K ( + )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Permeability and conductivity ratios were distinct for cells dialyzed with Na ( + ) - or K ( + ) - based internal solution , and application of external glutamate altered anion permeability ratios and the concentration dependence of the anion influx .
	manualset3
123413	5	405052	5	NULL	NULL	0	NULL	internal solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Permeability and conductivity ratios were distinct for cells dialyzed with Na ( + ) - or K ( + ) - based internal solution , and application of external glutamate altered anion permeability ratios and the concentration dependence of the anion influx .
	manualset3
123414	6	405052	5	NULL	NULL	0	NULL	application 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Permeability and conductivity ratios were distinct for cells dialyzed with Na ( + ) - or K ( + ) - based internal solution , and application of external glutamate altered anion permeability ratios and the concentration dependence of the anion influx .
	manualset3
123415	7	405052	5	NULL	NULL	0	NULL	external glutamate	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Permeability and conductivity ratios were distinct for cells dialyzed with Na ( + ) - or K ( + ) - based internal solution , and application of external glutamate altered anion permeability ratios and the concentration dependence of the anion influx .
	manualset3
123416	8	405052	5	NULL	NULL	0	NULL	anion permeability ratios 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Permeability and conductivity ratios were distinct for cells dialyzed with Na ( + ) - or K ( + ) - based internal solution , and application of external glutamate altered anion permeability ratios and the concentration dependence of the anion influx .
	manualset3
123417	9	405052	5	NULL	NULL	0	NULL	concentration dependence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Permeability and conductivity ratios were distinct for cells dialyzed with Na ( + ) - or K ( + ) - based internal solution , and application of external glutamate altered anion permeability ratios and the concentration dependence of the anion influx .
	manualset3
123418	10	405052	5	NULL	NULL	0	NULL	anion influx	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Permeability and conductivity ratios were distinct for cells dialyzed with Na ( + ) - or K ( + ) - based internal solution , and application of external glutamate altered anion permeability ratios and the concentration dependence of the anion influx .
	manualset3
123419	1	405053	5	NULL	NULL	0	NULL	Permeabilized acinar cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Permeabilized acinar cells rapidly accumulated Ca2 + to steady-state .
	manualset3
123420	2	405053	5	NULL	NULL	0	NULL	Ca2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Permeabilized acinar cells rapidly accumulated Ca2 + to steady-state .
	manualset3
123421	3	405053	5	NULL	NULL	0	NULL	steady-state	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Permeabilized acinar cells rapidly accumulated Ca2 + to steady-state .
	manualset3
123422	1	405054	5	NULL	NULL	0	NULL	Peroneal mononeuropathy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroneal mononeuropathy : predisposing factors , and clinical and neurophysiological relationships .
	manualset3
123423	2	405054	5	NULL	NULL	0	NULL	predisposing factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroneal mononeuropathy : predisposing factors , and clinical and neurophysiological relationships .
	manualset3
123424	3	405054	5	NULL	NULL	0	NULL	clinical relationships 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroneal mononeuropathy : predisposing factors , and clinical and neurophysiological relationships .
	manualset3
123425	4	405054	5	NULL	NULL	0	NULL	neurophysiological relationships 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroneal mononeuropathy : predisposing factors , and clinical and neurophysiological relationships .
	manualset3
123426	1	405055	5	NULL	NULL	0	NULL	statistical difference	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A greater statistical difference ( P less than 0.005 ) was found when the actuarial survival was analyzed in relation to the diffuse or nondiffuse pattern of bone marrow histology .
	manualset3
123427	2	405055	5	NULL	NULL	0	NULL	P less than 0.005	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A greater statistical difference ( P less than 0.005 ) was found when the actuarial survival was analyzed in relation to the diffuse or nondiffuse pattern of bone marrow histology .
	manualset3
123428	3	405055	5	NULL	NULL	0	NULL	actuarial survival 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A greater statistical difference ( P less than 0.005 ) was found when the actuarial survival was analyzed in relation to the diffuse or nondiffuse pattern of bone marrow histology .
	manualset3
123429	4	405055	5	NULL	NULL	0	NULL	relation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A greater statistical difference ( P less than 0.005 ) was found when the actuarial survival was analyzed in relation to the diffuse or nondiffuse pattern of bone marrow histology .
	manualset3
123430	5	405055	5	NULL	NULL	0	NULL	diffuse or nondiffuse pattern	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A greater statistical difference ( P less than 0.005 ) was found when the actuarial survival was analyzed in relation to the diffuse or nondiffuse pattern of bone marrow histology .
	manualset3
123431	6	405055	5	NULL	NULL	NULL	NULL	bone marrow histology	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A greater statistical difference ( P less than 0.005 ) was found when the actuarial survival was analyzed in relation to the diffuse or nondiffuse pattern of bone marrow histology .
	manualset3
123432	1	405056	5	NULL	NULL	0	NULL	Perosseous venography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Perosseous venography in the diagnosis of viability in subcapital fractures of the femur .
	manualset3
123433	2	405056	5	NULL	NULL	0	NULL	diagnosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Perosseous venography in the diagnosis of viability in subcapital fractures of the femur .
	manualset3
123434	3	405056	5	NULL	NULL	NULL	NULL	viability 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Perosseous venography in the diagnosis of viability in subcapital fractures of the femur .
	manualset3
123435	4	405056	5	NULL	NULL	0	NULL	subcapital fractures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Perosseous venography in the diagnosis of viability in subcapital fractures of the femur .
	manualset3
123436	5	405056	5	NULL	NULL	0	NULL	femur 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Perosseous venography in the diagnosis of viability in subcapital fractures of the femur .
	manualset3
123451	1	405057	5	NULL	NULL	0	NULL	Peroxiredoxin Q	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxiredoxin Q decomposes peroxides using thioredoxin as an electron donor with a substrate preference of H ( 2 ) O ( 2 ) ) cumene hydroperoxide ) ) butyl hydroperoxide ) ) linoleoyl hydroperoxide and insignificant affinity towards complex phospholipid hydroperoxide .
	manualset3
123456	2	405057	5	NULL	NULL	0	NULL	peroxides 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxiredoxin Q decomposes peroxides using thioredoxin as an electron donor with a substrate preference of H ( 2 ) O ( 2 ) ) cumene hydroperoxide ) ) butyl hydroperoxide ) ) linoleoyl hydroperoxide and insignificant affinity towards complex phospholipid hydroperoxide .
	manualset3
123463	3	405057	5	NULL	NULL	0	NULL	thioredoxin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxiredoxin Q decomposes peroxides using thioredoxin as an electron donor with a substrate preference of H ( 2 ) O ( 2 ) ) cumene hydroperoxide ) ) butyl hydroperoxide ) ) linoleoyl hydroperoxide and insignificant affinity towards complex phospholipid hydroperoxide .
	manualset3
123468	4	405057	5	NULL	NULL	0	NULL	electron donor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxiredoxin Q decomposes peroxides using thioredoxin as an electron donor with a substrate preference of H ( 2 ) O ( 2 ) ) cumene hydroperoxide ) ) butyl hydroperoxide ) ) linoleoyl hydroperoxide and insignificant affinity towards complex phospholipid hydroperoxide .
	manualset3
123469	5	405057	5	NULL	NULL	0	NULL	substrate preference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxiredoxin Q decomposes peroxides using thioredoxin as an electron donor with a substrate preference of H ( 2 ) O ( 2 ) ) cumene hydroperoxide ) ) butyl hydroperoxide ) ) linoleoyl hydroperoxide and insignificant affinity towards complex phospholipid hydroperoxide .
	manualset3
123477	6	405057	5	NULL	NULL	0	NULL	H(2)O(2)	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxiredoxin Q decomposes peroxides using thioredoxin as an electron donor with a substrate preference of H ( 2 ) O ( 2 ) ) cumene hydroperoxide ) ) butyl hydroperoxide ) ) linoleoyl hydroperoxide and insignificant affinity towards complex phospholipid hydroperoxide .
	manualset3
123479	7	405057	5	NULL	NULL	0	NULL	cumene hydroperoxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxiredoxin Q decomposes peroxides using thioredoxin as an electron donor with a substrate preference of H ( 2 ) O ( 2 ) ) cumene hydroperoxide ) ) butyl hydroperoxide ) ) linoleoyl hydroperoxide and insignificant affinity towards complex phospholipid hydroperoxide .
	manualset3
123481	8	405057	5	NULL	NULL	0	NULL	butyl hydroperoxide 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxiredoxin Q decomposes peroxides using thioredoxin as an electron donor with a substrate preference of H ( 2 ) O ( 2 ) ) cumene hydroperoxide ) ) butyl hydroperoxide ) ) linoleoyl hydroperoxide and insignificant affinity towards complex phospholipid hydroperoxide .
	manualset3
123483	9	405057	5	NULL	NULL	0	NULL	linoleoyl hydroperoxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxiredoxin Q decomposes peroxides using thioredoxin as an electron donor with a substrate preference of H ( 2 ) O ( 2 ) ) cumene hydroperoxide ) ) butyl hydroperoxide ) ) linoleoyl hydroperoxide and insignificant affinity towards complex phospholipid hydroperoxide .
	manualset3
123499	10	405057	5	NULL	NULL	0	NULL	affinity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxiredoxin Q decomposes peroxides using thioredoxin as an electron donor with a substrate preference of H ( 2 ) O ( 2 ) ) cumene hydroperoxide ) ) butyl hydroperoxide ) ) linoleoyl hydroperoxide and insignificant affinity towards complex phospholipid hydroperoxide .
	manualset3
123500	11	405057	5	NULL	NULL	0	NULL	complex phospholipid hydroperoxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxiredoxin Q decomposes peroxides using thioredoxin as an electron donor with a substrate preference of H ( 2 ) O ( 2 ) ) cumene hydroperoxide ) ) butyl hydroperoxide ) ) linoleoyl hydroperoxide and insignificant affinity towards complex phospholipid hydroperoxide .
	manualset3
123502	1	405058	5	NULL	NULL	0	NULL	Peroxisomal disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxisomal disorders : concentrations of metabolites in cerebrospinal fluid compared with plasma .
	manualset3
123504	2	405058	5	NULL	NULL	0	NULL	concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxisomal disorders : concentrations of metabolites in cerebrospinal fluid compared with plasma .
	manualset3
123506	3	405058	5	NULL	NULL	0	NULL	metabolites 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxisomal disorders : concentrations of metabolites in cerebrospinal fluid compared with plasma .
	manualset3
123510	4	405058	5	NULL	NULL	0	NULL	cerebrospinal fluid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxisomal disorders : concentrations of metabolites in cerebrospinal fluid compared with plasma .
	manualset3
123511	5	405058	5	NULL	NULL	0	NULL	plasma 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxisomal disorders : concentrations of metabolites in cerebrospinal fluid compared with plasma .
	manualset3
123517	1	405059	5	NULL	NULL	0	NULL	Peroxisome proliferator-activated receptor gamma ( PPARgamma )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxisome proliferator-activated receptor gamma ( PPARgamma ) is a member of the nuclear receptor superfamily of ligand-activated transcription factors and is expressed in several types of tissue .
	manualset3
123520	2	405059	5	NULL	NULL	0	NULL	member 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxisome proliferator-activated receptor gamma ( PPARgamma ) is a member of the nuclear receptor superfamily of ligand-activated transcription factors and is expressed in several types of tissue .
	manualset3
123521	3	405059	5	NULL	NULL	0	NULL	nuclear receptor superfamily 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxisome proliferator-activated receptor gamma ( PPARgamma ) is a member of the nuclear receptor superfamily of ligand-activated transcription factors and is expressed in several types of tissue .
	manualset3
123522	4	405059	5	NULL	NULL	0	NULL	ligand-activated transcription factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxisome proliferator-activated receptor gamma ( PPARgamma ) is a member of the nuclear receptor superfamily of ligand-activated transcription factors and is expressed in several types of tissue .
	manualset3
123523	5	405059	5	NULL	NULL	0	NULL	several types	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxisome proliferator-activated receptor gamma ( PPARgamma ) is a member of the nuclear receptor superfamily of ligand-activated transcription factors and is expressed in several types of tissue .
	manualset3
123524	6	405059	5	NULL	NULL	0	NULL	tissue 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxisome proliferator-activated receptor gamma ( PPARgamma ) is a member of the nuclear receptor superfamily of ligand-activated transcription factors and is expressed in several types of tissue .
	manualset3
123525	1	405060	5	NULL	NULL	0	NULL	Peroxisome proliferator-activated receptors ( PPARs )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxisome proliferator-activated receptors ( PPARs ) are nuclear transcription factors which are involved in many biological processes , such as regulation of cell differentiation , lipid metabolism , inflammation and cell death .
	manualset3
123526	2	405060	5	NULL	NULL	0	NULL	nuclear transcription factors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxisome proliferator-activated receptors ( PPARs ) are nuclear transcription factors which are involved in many biological processes , such as regulation of cell differentiation , lipid metabolism , inflammation and cell death .
	manualset3
123527	3	405060	5	NULL	NULL	0	NULL	biological processes 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxisome proliferator-activated receptors ( PPARs ) are nuclear transcription factors which are involved in many biological processes , such as regulation of cell differentiation , lipid metabolism , inflammation and cell death .
	manualset3
123529	4	405060	5	NULL	NULL	0	NULL	regulation of cell differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxisome proliferator-activated receptors ( PPARs ) are nuclear transcription factors which are involved in many biological processes , such as regulation of cell differentiation , lipid metabolism , inflammation and cell death .
	manualset3
123532	5	405060	5	NULL	NULL	0	NULL	lipid metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxisome proliferator-activated receptors ( PPARs ) are nuclear transcription factors which are involved in many biological processes , such as regulation of cell differentiation , lipid metabolism , inflammation and cell death .
	manualset3
123533	6	405060	5	NULL	NULL	0	NULL	inflammation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxisome proliferator-activated receptors ( PPARs ) are nuclear transcription factors which are involved in many biological processes , such as regulation of cell differentiation , lipid metabolism , inflammation and cell death .
	manualset3
123536	7	405060	5	NULL	NULL	0	NULL	cell death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxisome proliferator-activated receptors ( PPARs ) are nuclear transcription factors which are involved in many biological processes , such as regulation of cell differentiation , lipid metabolism , inflammation and cell death .
	manualset3
123542	1	405061	5	NULL	NULL	0	NULL	Peroxynitrite-mediated hepatic injury 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxynitrite-mediated hepatic injury in rats was induced by administration of galactosamine/lipopolysaccharide ( GalN/LPS ) .
	manualset3
123544	2	405061	5	NULL	NULL	0	NULL	rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxynitrite-mediated hepatic injury in rats was induced by administration of galactosamine/lipopolysaccharide ( GalN/LPS ) .
	manualset3
123546	3	405061	5	NULL	NULL	0	NULL	administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxynitrite-mediated hepatic injury in rats was induced by administration of galactosamine/lipopolysaccharide ( GalN/LPS ) .
	manualset3
123547	4	405061	5	NULL	NULL	0	NULL	galactosamine/lipopolysaccharide ( GalN/LPS )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxynitrite-mediated hepatic injury in rats was induced by administration of galactosamine/lipopolysaccharide ( GalN/LPS ) .
	manualset3
123609	1	405062	5	NULL	NULL	0	NULL	Peroxynitrite 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxynitrite induces covalent dimerization of epidermal growth factor receptors in A431 epidermoid carcinoma cells .
	manualset3
123610	2	405062	5	NULL	NULL	0	NULL	covalent dimerization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxynitrite induces covalent dimerization of epidermal growth factor receptors in A431 epidermoid carcinoma cells .
	manualset3
123611	3	405062	5	NULL	NULL	0	NULL	epidermal growth factor receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxynitrite induces covalent dimerization of epidermal growth factor receptors in A431 epidermoid carcinoma cells .
	manualset3
123612	4	405062	5	NULL	NULL	0	NULL	A431 epidermoid carcinoma cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Peroxynitrite induces covalent dimerization of epidermal growth factor receptors in A431 epidermoid carcinoma cells .
	manualset3
123613	1	405063	5	NULL	NULL	0	NULL	grid 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A grid of Au disks , 30 nm in diameter and 30 nm thick , is prepared on a SiO2 surface by conventional e-beam writing .
	manualset3
123614	2	405063	5	NULL	NULL	0	NULL	Au disks	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A grid of Au disks , 30 nm in diameter and 30 nm thick , is prepared on a SiO2 surface by conventional e-beam writing .
	manualset3
123615	3	405063	5	NULL	NULL	0	NULL	30 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A grid of Au disks , 30 nm in diameter and 30 nm thick , is prepared on a SiO2 surface by conventional e-beam writing .
	manualset3
123616	4	405063	5	NULL	NULL	0	NULL	diameter 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A grid of Au disks , 30 nm in diameter and 30 nm thick , is prepared on a SiO2 surface by conventional e-beam writing .
	manualset3
123617	5	405063	5	NULL	NULL	0	NULL	30 nm 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A grid of Au disks , 30 nm in diameter and 30 nm thick , is prepared on a SiO2 surface by conventional e-beam writing .
	manualset3
123618	6	405063	5	NULL	NULL	0	NULL	thick 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A grid of Au disks , 30 nm in diameter and 30 nm thick , is prepared on a SiO2 surface by conventional e-beam writing .
	manualset3
123619	7	405063	5	NULL	NULL	0	NULL	SiO2 surface 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A grid of Au disks , 30 nm in diameter and 30 nm thick , is prepared on a SiO2 surface by conventional e-beam writing .
	manualset3
123620	8	405063	5	NULL	NULL	0	NULL	conventional e-beam writing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A grid of Au disks , 30 nm in diameter and 30 nm thick , is prepared on a SiO2 surface by conventional e-beam writing .
	manualset3
123621	1	405064	5	NULL	NULL	0	NULL	Persistent pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Persistent pain , disability , and depression are hallmarks for chronic pain .
	manualset3
123622	2	405064	5	NULL	NULL	0	NULL	disability 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Persistent pain , disability , and depression are hallmarks for chronic pain .
	manualset3
123623	3	405064	5	NULL	NULL	0	NULL	depression 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Persistent pain , disability , and depression are hallmarks for chronic pain .
	manualset3
123624	4	405064	5	NULL	NULL	0	NULL	hallmarks 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Persistent pain , disability , and depression are hallmarks for chronic pain .
	manualset3
123625	5	405064	5	NULL	NULL	0	NULL	chronic pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Persistent pain , disability , and depression are hallmarks for chronic pain .
	manualset3
123626	1	405065	5	NULL	NULL	0	NULL	Personality characteristics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Personality characteristics in a sample of heroin addict methadone maintenance applicants .
	manualset3
123627	2	405065	5	NULL	NULL	0	NULL	sample 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Personality characteristics in a sample of heroin addict methadone maintenance applicants .
	manualset3
123628	3	405065	5	NULL	NULL	0	NULL	heroin addict methadone maintenance applicants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Personality characteristics in a sample of heroin addict methadone maintenance applicants .
	manualset3
123629	1	405066	5	NULL	NULL	NULL	NULL	Personality characteristics 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Personality characteristics of drug addicts and alcoholics on the Millon Clinical Multiaxial Inventory .
	manualset3
123630	2	405066	5	NULL	NULL	0	NULL	drug addicts	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Personality characteristics of drug addicts and alcoholics on the Millon Clinical Multiaxial Inventory .
	manualset3
123631	3	405066	5	NULL	NULL	0	NULL	alcoholics 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Personality characteristics of drug addicts and alcoholics on the Millon Clinical Multiaxial Inventory .
	manualset3
123632	4	405066	5	NULL	NULL	0	NULL	Millon Clinical Multiaxial Inventory	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Personality characteristics of drug addicts and alcoholics on the Millon Clinical Multiaxial Inventory .
	manualset3
123633	1	405067	5	NULL	NULL	0	NULL	Personality disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Personality disorders frequently occur as comorbid disorder in alcohol-dependent subjects .
	manualset3
123634	2	405067	5	NULL	NULL	0	NULL	comorbid disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Personality disorders frequently occur as comorbid disorder in alcohol-dependent subjects .
	manualset3
123635	3	405067	5	NULL	NULL	0	NULL	alcohol-dependent subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Personality disorders frequently occur as comorbid disorder in alcohol-dependent subjects .
	manualset3
123636	1	405068	5	NULL	NULL	NULL	NULL	Personality traits 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Personality traits and psychophysiological reactions to a stressful interview in twins with varying degrees of coronary heart disease .
	manualset3
123637	2	405068	5	NULL	NULL	0	NULL	psychophysiological reactions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Personality traits and psychophysiological reactions to a stressful interview in twins with varying degrees of coronary heart disease .
	manualset3
123638	3	405068	5	NULL	NULL	0	NULL	stressful interview	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Personality traits and psychophysiological reactions to a stressful interview in twins with varying degrees of coronary heart disease .
	manualset3
123639	4	405068	5	NULL	NULL	0	NULL	twins 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Personality traits and psychophysiological reactions to a stressful interview in twins with varying degrees of coronary heart disease .
	manualset3
123640	5	405068	5	NULL	NULL	0	NULL	varying degrees 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Personality traits and psychophysiological reactions to a stressful interview in twins with varying degrees of coronary heart disease .
	manualset3
123641	6	405068	5	NULL	NULL	0	NULL	coronary heart disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Personality traits and psychophysiological reactions to a stressful interview in twins with varying degrees of coronary heart disease .
	manualset3
123642	1	405069	5	NULL	NULL	0	NULL	Persons 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Persons diagnosed at earlier stages incurred higher total payments between diagnosis and death than those diagnosed at later stages , reflecting their longer survival .
	manualset3
123643	2	405069	5	NULL	NULL	NULL	NULL	earlier stages 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Persons diagnosed at earlier stages incurred higher total payments between diagnosis and death than those diagnosed at later stages , reflecting their longer survival .
	manualset3
123644	3	405069	5	NULL	NULL	0	NULL	higher total payments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Persons diagnosed at earlier stages incurred higher total payments between diagnosis and death than those diagnosed at later stages , reflecting their longer survival .
	manualset3
123645	4	405069	5	NULL	NULL	0	NULL	diagnosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Persons diagnosed at earlier stages incurred higher total payments between diagnosis and death than those diagnosed at later stages , reflecting their longer survival .
	manualset3
123646	5	405069	5	NULL	NULL	0	NULL	death 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Persons diagnosed at earlier stages incurred higher total payments between diagnosis and death than those diagnosed at later stages , reflecting their longer survival .
	manualset3
123647	6	405069	5	NULL	NULL	0	NULL	 later stages	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Persons diagnosed at earlier stages incurred higher total payments between diagnosis and death than those diagnosed at later stages , reflecting their longer survival .
	manualset3
123648	7	405069	5	NULL	NULL	0	NULL	longer survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Persons diagnosed at earlier stages incurred higher total payments between diagnosis and death than those diagnosed at later stages , reflecting their longer survival .
	manualset3
123649	1	405070	5	NULL	NULL	0	NULL	Persons 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Persons for whom vaccination is recommended are listed in boxes 1 and 2 .
	manualset3
123650	2	405070	5	NULL	NULL	0	NULL	vaccination 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Persons for whom vaccination is recommended are listed in boxes 1 and 2 .
	manualset3
123652	3	405070	5	NULL	NULL	NULL	NULL	box 1	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Persons for whom vaccination is recommended are listed in boxes 1 and 2 .
	manualset3
123653	4	405070	5	NULL	NULL	0	NULL	box 2	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Persons for whom vaccination is recommended are listed in boxes 1 and 2 .
	manualset3
123654	1	405071	5	NULL	NULL	0	NULL	Pertinent ongoing interventions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pertinent ongoing interventions ( delaying early child birth , adequate antenatal care and maternal iron-folate supplementation ) are beneficial but have sub-optimal coverage .
	manualset3
123655	2	405071	5	NULL	NULL	0	NULL	early child birth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pertinent ongoing interventions ( delaying early child birth , adequate antenatal care and maternal iron-folate supplementation ) are beneficial but have sub-optimal coverage .
	manualset3
123656	3	405071	5	NULL	NULL	0	NULL	adequate antenatal care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pertinent ongoing interventions ( delaying early child birth , adequate antenatal care and maternal iron-folate supplementation ) are beneficial but have sub-optimal coverage .
	manualset3
123657	4	405071	5	NULL	NULL	0	NULL	maternal iron-folate supplementation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pertinent ongoing interventions ( delaying early child birth , adequate antenatal care and maternal iron-folate supplementation ) are beneficial but have sub-optimal coverage .
	manualset3
123658	5	405071	5	NULL	NULL	0	NULL	sub-optimal coverage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pertinent ongoing interventions ( delaying early child birth , adequate antenatal care and maternal iron-folate supplementation ) are beneficial but have sub-optimal coverage .
	manualset3
123659	1	405072	5	NULL	NULL	0	NULL	Perturbation studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Perturbation studies revealed that pH shifts from 7.2 to 7.5 decreased TCE degradation by 85 % .
	manualset3
123660	2	405072	5	NULL	NULL	0	NULL	 pH shifts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Perturbation studies revealed that pH shifts from 7.2 to 7.5 decreased TCE degradation by 85 % .
	manualset3
123661	3	405072	5	NULL	NULL	0	NULL	7.2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Perturbation studies revealed that pH shifts from 7.2 to 7.5 decreased TCE degradation by 85 % .
	manualset3
123662	4	405072	5	NULL	NULL	0	NULL	7.5	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Perturbation studies revealed that pH shifts from 7.2 to 7.5 decreased TCE degradation by 85 % .
	manualset3
123663	5	405072	5	NULL	NULL	0	NULL	TCE degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Perturbation studies revealed that pH shifts from 7.2 to 7.5 decreased TCE degradation by 85 % .
	manualset3
123664	6	405072	5	NULL	NULL	0	NULL	85 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Perturbation studies revealed that pH shifts from 7.2 to 7.5 decreased TCE degradation by 85 % .
	manualset3
123665	1	405073	5	NULL	NULL	0	NULL	Perturbations 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Perturbations imposed on such computer simulations caused catastrophic breakdowns of neural functioning .
	manualset3
123666	2	405073	5	NULL	NULL	0	NULL	computer simulations 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Perturbations imposed on such computer simulations caused catastrophic breakdowns of neural functioning .
	manualset3
123667	3	405073	5	NULL	NULL	0	NULL	catastrophic breakdowns 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Perturbations imposed on such computer simulations caused catastrophic breakdowns of neural functioning .
	manualset3
123668	4	405073	5	NULL	NULL	0	NULL	neural functioning	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Perturbations imposed on such computer simulations caused catastrophic breakdowns of neural functioning .
	manualset3
123669	1	405074	5	NULL	NULL	0	NULL	Pesticide residues	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Pesticide residues on the external surfaces of field-crop sprayers : environmental impact .
	manualset3
123670	2	405074	5	NULL	NULL	0	NULL	external surfaces 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pesticide residues on the external surfaces of field-crop sprayers : environmental impact .
	manualset3
123671	3	405074	5	NULL	NULL	0	NULL	field-crop sprayers	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Pesticide residues on the external surfaces of field-crop sprayers : environmental impact .
	manualset3
123672	4	405074	5	NULL	NULL	0	NULL	environmental impact 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pesticide residues on the external surfaces of field-crop sprayers : environmental impact .
	manualset3
123673	1	405075	5	NULL	NULL	0	NULL	Phage M102AD 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Phage M102AD adsorbed very slowly to its host , and it can not adsorb to serotype e and f strains of S. mutans .
	manualset3
123674	2	405075	5	NULL	NULL	0	NULL	host 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Phage M102AD adsorbed very slowly to its host , and it can not adsorb to serotype e and f strains of S. mutans .
	manualset3
123675	3	405075	5	NULL	NULL	0	NULL	serotype e strain of S. mutans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Phage M102AD adsorbed very slowly to its host , and it can not adsorb to serotype e and f strains of S. mutans .
	manualset3
123676	4	405075	5	NULL	NULL	0	NULL	serotype f strains of S. mutans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Phage M102AD adsorbed very slowly to its host , and it can not adsorb to serotype e and f strains of S. mutans .
	manualset3
123677	1	405076	5	NULL	NULL	0	NULL	Phagocytic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Phagocytic activity of neuronal progenitors regulates adult neurogenesis .
	manualset3
123678	2	405076	5	NULL	NULL	0	NULL	neuronal progenitors	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Phagocytic activity of neuronal progenitors regulates adult neurogenesis .
	manualset3
123679	3	405076	5	NULL	NULL	0	NULL	adult neurogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Phagocytic activity of neuronal progenitors regulates adult neurogenesis .
	manualset3
123680	1	405077	5	NULL	NULL	0	NULL	group 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A group of 19 acyclic terpenes have been evaluated for potential toxicity/carcinogenicity by molecular orbital determinations of their spatial and electronic parameters , and hence prediction of their metabolic activation or detoxication by the cytochrome P-450 ( CYP ) superfamily of mixed-function oxidase enzymes .
	manualset3
123681	2	405077	5	NULL	NULL	0	NULL	19 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A group of 19 acyclic terpenes have been evaluated for potential toxicity/carcinogenicity by molecular orbital determinations of their spatial and electronic parameters , and hence prediction of their metabolic activation or detoxication by the cytochrome P-450 ( CYP ) superfamily of mixed-function oxidase enzymes .
	manualset3
123682	3	405077	5	NULL	NULL	0	NULL	acyclic terpenes	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A group of 19 acyclic terpenes have been evaluated for potential toxicity/carcinogenicity by molecular orbital determinations of their spatial and electronic parameters , and hence prediction of their metabolic activation or detoxication by the cytochrome P-450 ( CYP ) superfamily of mixed-function oxidase enzymes .
	manualset3
123683	4	405077	5	NULL	NULL	0	NULL	potential toxicity/carcinogenicity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A group of 19 acyclic terpenes have been evaluated for potential toxicity/carcinogenicity by molecular orbital determinations of their spatial and electronic parameters , and hence prediction of their metabolic activation or detoxication by the cytochrome P-450 ( CYP ) superfamily of mixed-function oxidase enzymes .
	manualset3
123684	5	405077	5	NULL	NULL	0	NULL	molecular orbital determinations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A group of 19 acyclic terpenes have been evaluated for potential toxicity/carcinogenicity by molecular orbital determinations of their spatial and electronic parameters , and hence prediction of their metabolic activation or detoxication by the cytochrome P-450 ( CYP ) superfamily of mixed-function oxidase enzymes .
	manualset3
123685	6	405077	5	NULL	NULL	0	NULL	spatial parameters	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A group of 19 acyclic terpenes have been evaluated for potential toxicity/carcinogenicity by molecular orbital determinations of their spatial and electronic parameters , and hence prediction of their metabolic activation or detoxication by the cytochrome P-450 ( CYP ) superfamily of mixed-function oxidase enzymes .
	manualset3
123686	7	405077	5	NULL	NULL	0	NULL	electronic parameters	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A group of 19 acyclic terpenes have been evaluated for potential toxicity/carcinogenicity by molecular orbital determinations of their spatial and electronic parameters , and hence prediction of their metabolic activation or detoxication by the cytochrome P-450 ( CYP ) superfamily of mixed-function oxidase enzymes .
	manualset3
123687	8	405077	5	NULL	NULL	0	NULL	prediction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A group of 19 acyclic terpenes have been evaluated for potential toxicity/carcinogenicity by molecular orbital determinations of their spatial and electronic parameters , and hence prediction of their metabolic activation or detoxication by the cytochrome P-450 ( CYP ) superfamily of mixed-function oxidase enzymes .
	manualset3
123688	9	405077	5	NULL	NULL	0	NULL	metabolic activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A group of 19 acyclic terpenes have been evaluated for potential toxicity/carcinogenicity by molecular orbital determinations of their spatial and electronic parameters , and hence prediction of their metabolic activation or detoxication by the cytochrome P-450 ( CYP ) superfamily of mixed-function oxidase enzymes .
	manualset3
123689	10	405077	5	NULL	NULL	0	NULL	detoxication 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A group of 19 acyclic terpenes have been evaluated for potential toxicity/carcinogenicity by molecular orbital determinations of their spatial and electronic parameters , and hence prediction of their metabolic activation or detoxication by the cytochrome P-450 ( CYP ) superfamily of mixed-function oxidase enzymes .
	manualset3
123690	11	405077	5	NULL	NULL	0	NULL	cytochrome P-450 ( CYP ) superfamily 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A group of 19 acyclic terpenes have been evaluated for potential toxicity/carcinogenicity by molecular orbital determinations of their spatial and electronic parameters , and hence prediction of their metabolic activation or detoxication by the cytochrome P-450 ( CYP ) superfamily of mixed-function oxidase enzymes .
	manualset3
123691	12	405077	5	NULL	NULL	0	NULL	mixed-function oxidase enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A group of 19 acyclic terpenes have been evaluated for potential toxicity/carcinogenicity by molecular orbital determinations of their spatial and electronic parameters , and hence prediction of their metabolic activation or detoxication by the cytochrome P-450 ( CYP ) superfamily of mixed-function oxidase enzymes .
	manualset3
123692	1	405078	5	NULL	NULL	0	NULL	Pharmacist support	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacist support for selling syringes without a prescription to injection drug users in Rhode Island .
	manualset3
123693	2	405078	5	NULL	NULL	0	NULL	syringes 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacist support for selling syringes without a prescription to injection drug users in Rhode Island .
	manualset3
123694	3	405078	5	NULL	NULL	0	NULL	prescription 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacist support for selling syringes without a prescription to injection drug users in Rhode Island .
	manualset3
123695	4	405078	5	NULL	NULL	0	NULL	injection drug users	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacist support for selling syringes without a prescription to injection drug users in Rhode Island .
	manualset3
123696	5	405078	5	NULL	NULL	0	NULL	Rhode Island	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacist support for selling syringes without a prescription to injection drug users in Rhode Island .
	manualset3
123697	1	405079	5	NULL	NULL	0	NULL	Pharmacogenetic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacogenetic analysis of human steroid 5 alpha reductase type II : comparison of finasteride and dutasteride .
	manualset3
123698	2	405079	5	NULL	NULL	0	NULL	human steroid 5 alpha reductase type II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacogenetic analysis of human steroid 5 alpha reductase type II : comparison of finasteride and dutasteride .
	manualset3
123699	3	405079	5	NULL	NULL	0	NULL	comparison 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacogenetic analysis of human steroid 5 alpha reductase type II : comparison of finasteride and dutasteride .
	manualset3
123700	4	405079	5	NULL	NULL	0	NULL	finasteride 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacogenetic analysis of human steroid 5 alpha reductase type II : comparison of finasteride and dutasteride .
	manualset3
123701	5	405079	5	NULL	NULL	0	NULL	dutasteride 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacogenetic analysis of human steroid 5 alpha reductase type II : comparison of finasteride and dutasteride .
	manualset3
123702	1	405080	5	NULL	NULL	0	NULL	Pharmacokinetic investigation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetic investigation Peak plasma concentrations of SY5555 after dose of 5 mg/kg , 10 mg/kg and 15 mg/kg were , respectively , 1.58 + / - 0.37 micrograms/ml , 2.78 + / - 0.54 micrograms/ml and 5.28 micrograms/ml at 1 hour .
	manualset3
123703	2	405080	5	NULL	NULL	0	NULL	Peak plasma concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetic investigation Peak plasma concentrations of SY5555 after dose of 5 mg/kg , 10 mg/kg and 15 mg/kg were , respectively , 1.58 + / - 0.37 micrograms/ml , 2.78 + / - 0.54 micrograms/ml and 5.28 micrograms/ml at 1 hour .
	manualset3
123704	3	405080	5	NULL	NULL	0	NULL	SY5555 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetic investigation Peak plasma concentrations of SY5555 after dose of 5 mg/kg , 10 mg/kg and 15 mg/kg were , respectively , 1.58 + / - 0.37 micrograms/ml , 2.78 + / - 0.54 micrograms/ml and 5.28 micrograms/ml at 1 hour .
	manualset3
123705	4	405080	5	NULL	NULL	0	NULL	dose 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetic investigation Peak plasma concentrations of SY5555 after dose of 5 mg/kg , 10 mg/kg and 15 mg/kg were , respectively , 1.58 + / - 0.37 micrograms/ml , 2.78 + / - 0.54 micrograms/ml and 5.28 micrograms/ml at 1 hour .
	manualset3
123706	5	405080	5	NULL	NULL	0	NULL	5 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetic investigation Peak plasma concentrations of SY5555 after dose of 5 mg/kg , 10 mg/kg and 15 mg/kg were , respectively , 1.58 + / - 0.37 micrograms/ml , 2.78 + / - 0.54 micrograms/ml and 5.28 micrograms/ml at 1 hour .
	manualset3
123707	6	405080	5	NULL	NULL	0	NULL	10 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetic investigation Peak plasma concentrations of SY5555 after dose of 5 mg/kg , 10 mg/kg and 15 mg/kg were , respectively , 1.58 + / - 0.37 micrograms/ml , 2.78 + / - 0.54 micrograms/ml and 5.28 micrograms/ml at 1 hour .
	manualset3
123708	7	405080	5	NULL	NULL	0	NULL	15 mg/kg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetic investigation Peak plasma concentrations of SY5555 after dose of 5 mg/kg , 10 mg/kg and 15 mg/kg were , respectively , 1.58 + / - 0.37 micrograms/ml , 2.78 + / - 0.54 micrograms/ml and 5.28 micrograms/ml at 1 hour .
	manualset3
123709	8	405080	5	NULL	NULL	0	NULL	1.58 + / - 0.37 micrograms/ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetic investigation Peak plasma concentrations of SY5555 after dose of 5 mg/kg , 10 mg/kg and 15 mg/kg were , respectively , 1.58 + / - 0.37 micrograms/ml , 2.78 + / - 0.54 micrograms/ml and 5.28 micrograms/ml at 1 hour .
	manualset3
123710	9	405080	5	NULL	NULL	0	NULL	2.78 + / - 0.54 micrograms/ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetic investigation Peak plasma concentrations of SY5555 after dose of 5 mg/kg , 10 mg/kg and 15 mg/kg were , respectively , 1.58 + / - 0.37 micrograms/ml , 2.78 + / - 0.54 micrograms/ml and 5.28 micrograms/ml at 1 hour .
	manualset3
123711	10	405080	5	NULL	NULL	0	NULL	5.28 micrograms/ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetic investigation Peak plasma concentrations of SY5555 after dose of 5 mg/kg , 10 mg/kg and 15 mg/kg were , respectively , 1.58 + / - 0.37 micrograms/ml , 2.78 + / - 0.54 micrograms/ml and 5.28 micrograms/ml at 1 hour .
	manualset3
123712	11	405080	5	NULL	NULL	0	NULL	1 hour	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetic investigation Peak plasma concentrations of SY5555 after dose of 5 mg/kg , 10 mg/kg and 15 mg/kg were , respectively , 1.58 + / - 0.37 micrograms/ml , 2.78 + / - 0.54 micrograms/ml and 5.28 micrograms/ml at 1 hour .
	manualset3
123713	1	405081	5	NULL	NULL	0	NULL	Pharmacokinetic study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetic study of gemcitabine , given as prolonged infusion at fixed dose rate , in combination with cisplatin in patients with advanced non-small-cell lung cancer .
	manualset3
123714	2	405081	5	NULL	NULL	0	NULL	gemcitabine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetic study of gemcitabine , given as prolonged infusion at fixed dose rate , in combination with cisplatin in patients with advanced non-small-cell lung cancer .
	manualset3
123715	3	405081	5	NULL	NULL	0	NULL	prolonged infusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetic study of gemcitabine , given as prolonged infusion at fixed dose rate , in combination with cisplatin in patients with advanced non-small-cell lung cancer .
	manualset3
123716	4	405081	5	NULL	NULL	0	NULL	fixed dose rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetic study of gemcitabine , given as prolonged infusion at fixed dose rate , in combination with cisplatin in patients with advanced non-small-cell lung cancer .
	manualset3
123717	5	405081	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetic study of gemcitabine , given as prolonged infusion at fixed dose rate , in combination with cisplatin in patients with advanced non-small-cell lung cancer .
	manualset3
123718	6	405081	5	NULL	NULL	0	NULL	cisplatin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetic study of gemcitabine , given as prolonged infusion at fixed dose rate , in combination with cisplatin in patients with advanced non-small-cell lung cancer .
	manualset3
123719	7	405081	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetic study of gemcitabine , given as prolonged infusion at fixed dose rate , in combination with cisplatin in patients with advanced non-small-cell lung cancer .
	manualset3
123720	8	405081	5	NULL	NULL	0	NULL	advanced non-small-cell lung cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetic study of gemcitabine , given as prolonged infusion at fixed dose rate , in combination with cisplatin in patients with advanced non-small-cell lung cancer .
	manualset3
123721	1	405082	5	NULL	NULL	0	NULL	Pharmacokinetics 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetics and biotransformation of benzbromarone in man .
	manualset3
123722	2	405082	5	NULL	NULL	0	NULL	biotransformation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetics and biotransformation of benzbromarone in man .
	manualset3
123723	3	405082	5	NULL	NULL	0	NULL	benzbromarone 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetics and biotransformation of benzbromarone in man .
	manualset3
123724	4	405082	5	NULL	NULL	0	NULL	man 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetics and biotransformation of benzbromarone in man .
	manualset3
123725	1	405083	5	NULL	NULL	0	NULL	Pharmacokinetics 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetics of gabapentin in horses .
	manualset3
123726	2	405083	5	NULL	NULL	0	NULL	gabapentin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetics of gabapentin in horses .
	manualset3
123727	3	405083	5	NULL	NULL	0	NULL	horses 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetics of gabapentin in horses .
	manualset3
123728	1	405084	5	NULL	NULL	0	NULL	Pharmacokinetics 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetics of pirenzepine in patients with gastric or duodenal ulcers .
	manualset3
123729	2	405084	5	NULL	NULL	0	NULL	pirenzepine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetics of pirenzepine in patients with gastric or duodenal ulcers .
	manualset3
123730	3	405084	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetics of pirenzepine in patients with gastric or duodenal ulcers .
	manualset3
123731	4	405084	5	NULL	NULL	0	NULL	gastric ulcer	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetics of pirenzepine in patients with gastric or duodenal ulcers .
	manualset3
123732	5	405084	5	NULL	NULL	0	NULL	duodenal ulcer	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetics of pirenzepine in patients with gastric or duodenal ulcers .
	manualset3
123733	1	405085	5	NULL	NULL	0	NULL	group 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A group of middle-aged men ( n = 2322 ) were examined at a health screening which included an intravenous glucose tolerance test ( IVGTT ) with insulin determinations , and were then re-examined approximately 10 years later .
	manualset3
123734	2	405085	5	NULL	NULL	0	NULL	middle-aged men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A group of middle-aged men ( n = 2322 ) were examined at a health screening which included an intravenous glucose tolerance test ( IVGTT ) with insulin determinations , and were then re-examined approximately 10 years later .
	manualset3
123735	3	405085	5	NULL	NULL	0	NULL	n = 2322	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A group of middle-aged men ( n = 2322 ) were examined at a health screening which included an intravenous glucose tolerance test ( IVGTT ) with insulin determinations , and were then re-examined approximately 10 years later .
	manualset3
123736	4	405085	5	NULL	NULL	0	NULL	health screening 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A group of middle-aged men ( n = 2322 ) were examined at a health screening which included an intravenous glucose tolerance test ( IVGTT ) with insulin determinations , and were then re-examined approximately 10 years later .
	manualset3
123737	5	405085	5	NULL	NULL	0	NULL	intravenous glucose tolerance test ( IVGTT )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A group of middle-aged men ( n = 2322 ) were examined at a health screening which included an intravenous glucose tolerance test ( IVGTT ) with insulin determinations , and were then re-examined approximately 10 years later .
	manualset3
123738	6	405085	5	NULL	NULL	0	NULL	insulin determinations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A group of middle-aged men ( n = 2322 ) were examined at a health screening which included an intravenous glucose tolerance test ( IVGTT ) with insulin determinations , and were then re-examined approximately 10 years later .
	manualset3
123739	7	405085	5	NULL	NULL	0	NULL	10 year	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A group of middle-aged men ( n = 2322 ) were examined at a health screening which included an intravenous glucose tolerance test ( IVGTT ) with insulin determinations , and were then re-examined approximately 10 years later .
	manualset3
123740	1	405086	5	NULL	NULL	0	NULL	Pharmacological investigations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacological investigations of benzothiazoline derivatives .
	manualset3
123741	2	405086	5	NULL	NULL	0	NULL	benzothiazoline derivatives	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacological investigations of benzothiazoline derivatives .
	manualset3
123742	1	405087	5	NULL	NULL	0	NULL	Pharmacological treatments	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacological treatments , which block the dopamine system , are effective for delusions and hallucinations but less so for disabling cognitive and motivational impairments .
	manualset3
123743	2	405087	5	NULL	NULL	0	NULL	dopamine system	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacological treatments , which block the dopamine system , are effective for delusions and hallucinations but less so for disabling cognitive and motivational impairments .
	manualset3
123744	3	405087	5	NULL	NULL	0	NULL	delusions 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacological treatments , which block the dopamine system , are effective for delusions and hallucinations but less so for disabling cognitive and motivational impairments .
	manualset3
123745	4	405087	5	NULL	NULL	0	NULL	hallucinations 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacological treatments , which block the dopamine system , are effective for delusions and hallucinations but less so for disabling cognitive and motivational impairments .
	manualset3
123746	5	405087	5	NULL	NULL	0	NULL	cognitive impairments 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacological treatments , which block the dopamine system , are effective for delusions and hallucinations but less so for disabling cognitive and motivational impairments .
	manualset3
123747	6	405087	5	NULL	NULL	0	NULL	 motivational impairments 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacological treatments , which block the dopamine system , are effective for delusions and hallucinations but less so for disabling cognitive and motivational impairments .
	manualset3
123748	1	405088	5	NULL	NULL	0	NULL	Pharmacy education	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacy education and health planning .
	manualset3
123749	2	405088	5	NULL	NULL	0	NULL	health planning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacy education and health planning .
	manualset3
123750	1	405089	5	NULL	NULL	0	NULL	Pharyngeal tuberculosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharyngeal tuberculosis is an uncommon condition .
	manualset3
123751	2	405089	5	NULL	NULL	0	NULL	uncommon condition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharyngeal tuberculosis is an uncommon condition .
	manualset3
123752	1	405090	5	NULL	NULL	0	NULL	Phase I-II clinical studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase I-II clinical studies using PIXY321 are preliminary but show encouraging results with stimulation of multilineage hematopoiesis .
	manualset3
123753	2	405090	5	NULL	NULL	0	NULL	PIXY321	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase I-II clinical studies using PIXY321 are preliminary but show encouraging results with stimulation of multilineage hematopoiesis .
	manualset3
123754	3	405090	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase I-II clinical studies using PIXY321 are preliminary but show encouraging results with stimulation of multilineage hematopoiesis .
	manualset3
123755	4	405090	5	NULL	NULL	0	NULL	stimulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase I-II clinical studies using PIXY321 are preliminary but show encouraging results with stimulation of multilineage hematopoiesis .
	manualset3
123756	5	405090	5	NULL	NULL	0	NULL	multilineage hematopoiesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase I-II clinical studies using PIXY321 are preliminary but show encouraging results with stimulation of multilineage hematopoiesis .
	manualset3
123757	1	405091	5	NULL	NULL	0	NULL	Phase I clinical studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase I clinical studies confirmed that calcitriol 3 microg g ( -1 ) ointment is well tolerated in humans .
	manualset3
123758	2	405091	5	NULL	NULL	0	NULL	calcitriol 3 microg g ( -1 ) ointment	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase I clinical studies confirmed that calcitriol 3 microg g ( -1 ) ointment is well tolerated in humans .
	manualset3
123759	3	405091	5	NULL	NULL	0	NULL	humans 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase I clinical studies confirmed that calcitriol 3 microg g ( -1 ) ointment is well tolerated in humans .
	manualset3
123760	1	405092	5	NULL	NULL	0	NULL	Phase II study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase II study of vinorelbine in the treatment of platinum-resistant ovarian carcinoma .
	manualset3
123761	2	405092	5	NULL	NULL	0	NULL	vinorelbine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase II study of vinorelbine in the treatment of platinum-resistant ovarian carcinoma .
	manualset3
123762	3	405092	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase II study of vinorelbine in the treatment of platinum-resistant ovarian carcinoma .
	manualset3
123763	4	405092	5	NULL	NULL	0	NULL	platinum-resistant ovarian carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase II study of vinorelbine in the treatment of platinum-resistant ovarian carcinoma .
	manualset3
123764	1	405093	5	NULL	NULL	0	NULL	Phase II trial	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase II trial of i.v. vinorelbine and cisplatin in inoperable locally advanced or disseminated non-small-cell lung cancer : the South African experience .
	manualset3
123765	2	405093	5	NULL	NULL	0	NULL	i.v. vinorelbine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase II trial of i.v. vinorelbine and cisplatin in inoperable locally advanced or disseminated non-small-cell lung cancer : the South African experience .
	manualset3
123767	3	405093	5	NULL	NULL	0	NULL	cisplatin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase II trial of i.v. vinorelbine and cisplatin in inoperable locally advanced or disseminated non-small-cell lung cancer : the South African experience .
	manualset3
123768	4	405093	5	NULL	NULL	0	NULL	inoperable locally advanced or disseminated non-small-cell lung cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase II trial of i.v. vinorelbine and cisplatin in inoperable locally advanced or disseminated non-small-cell lung cancer : the South African experience .
	manualset3
123769	5	405093	5	NULL	NULL	0	NULL	South African experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase II trial of i.v. vinorelbine and cisplatin in inoperable locally advanced or disseminated non-small-cell lung cancer : the South African experience .
	manualset3
123770	1	405094	5	NULL	NULL	0	NULL	Phase II trials	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase II trials of erlotinib or gefitinib in patients with recurrent meningioma .
	manualset3
123771	2	405094	5	NULL	NULL	0	NULL	erlotinib 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase II trials of erlotinib or gefitinib in patients with recurrent meningioma .
	manualset3
123772	3	405094	5	NULL	NULL	0	NULL	gefitinib 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase II trials of erlotinib or gefitinib in patients with recurrent meningioma .
	manualset3
123773	4	405094	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase II trials of erlotinib or gefitinib in patients with recurrent meningioma .
	manualset3
123774	5	405094	5	NULL	NULL	0	NULL	recurrent meningioma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase II trials of erlotinib or gefitinib in patients with recurrent meningioma .
	manualset3
123775	1	405095	5	NULL	NULL	0	NULL	group 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A group of seven children who presented the encephalitic type of the illness and were hospitalized with symptoms of CNS involvement and a confirmed diagnosis of VEE constituted the index group .
	manualset3
123776	2	405095	5	NULL	NULL	0	NULL	seven 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A group of seven children who presented the encephalitic type of the illness and were hospitalized with symptoms of CNS involvement and a confirmed diagnosis of VEE constituted the index group .
	manualset3
123777	3	405095	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A group of seven children who presented the encephalitic type of the illness and were hospitalized with symptoms of CNS involvement and a confirmed diagnosis of VEE constituted the index group .
	manualset3
123778	4	405095	5	NULL	NULL	0	NULL	encephalitic type of the illness	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A group of seven children who presented the encephalitic type of the illness and were hospitalized with symptoms of CNS involvement and a confirmed diagnosis of VEE constituted the index group .
	manualset3
123779	5	405095	5	NULL	NULL	0	NULL	symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A group of seven children who presented the encephalitic type of the illness and were hospitalized with symptoms of CNS involvement and a confirmed diagnosis of VEE constituted the index group .
	manualset3
123780	6	405095	5	NULL	NULL	0	NULL	CNS involvement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A group of seven children who presented the encephalitic type of the illness and were hospitalized with symptoms of CNS involvement and a confirmed diagnosis of VEE constituted the index group .
	manualset3
123781	7	405095	5	NULL	NULL	0	NULL	confirmed diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A group of seven children who presented the encephalitic type of the illness and were hospitalized with symptoms of CNS involvement and a confirmed diagnosis of VEE constituted the index group .
	manualset3
123782	8	405095	5	NULL	NULL	0	NULL	VEE 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A group of seven children who presented the encephalitic type of the illness and were hospitalized with symptoms of CNS involvement and a confirmed diagnosis of VEE constituted the index group .
	manualset3
123783	9	405095	5	NULL	NULL	0	NULL	index group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A group of seven children who presented the encephalitic type of the illness and were hospitalized with symptoms of CNS involvement and a confirmed diagnosis of VEE constituted the index group .
	manualset3
123784	1	405096	5	NULL	NULL	0	NULL	Phase differences	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase differences between the navigator and image k-space data are used as an estimate of motion-induced phase shifts in the image , followed by autocorrection .
	manualset3
123785	2	405096	5	NULL	NULL	0	NULL	navigator 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase differences between the navigator and image k-space data are used as an estimate of motion-induced phase shifts in the image , followed by autocorrection .
	manualset3
123786	3	405096	5	NULL	NULL	0	NULL	image k-space data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase differences between the navigator and image k-space data are used as an estimate of motion-induced phase shifts in the image , followed by autocorrection .
	manualset3
123787	4	405096	5	NULL	NULL	0	NULL	estimate 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase differences between the navigator and image k-space data are used as an estimate of motion-induced phase shifts in the image , followed by autocorrection .
	manualset3
123788	5	405096	5	NULL	NULL	0	NULL	motion-induced phase shifts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase differences between the navigator and image k-space data are used as an estimate of motion-induced phase shifts in the image , followed by autocorrection .
	manualset3
123789	6	405096	5	NULL	NULL	0	NULL	image 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase differences between the navigator and image k-space data are used as an estimate of motion-induced phase shifts in the image , followed by autocorrection .
	manualset3
123790	7	405096	5	NULL	NULL	0	NULL	autocorrection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase differences between the navigator and image k-space data are used as an estimate of motion-induced phase shifts in the image , followed by autocorrection .
	manualset3
123791	1	405097	5	NULL	NULL	0	NULL	Phase 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase of Ising spins on modular networks analogous to social polarization .
	manualset3
123792	2	405097	5	NULL	NULL	0	NULL	Ising spins	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase of Ising spins on modular networks analogous to social polarization .
	manualset3
123793	3	405097	5	NULL	NULL	0	NULL	modular networks	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase of Ising spins on modular networks analogous to social polarization .
	manualset3
123794	4	405097	5	NULL	NULL	0	NULL	social polarization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Phase of Ising spins on modular networks analogous to social polarization .
	manualset3
123795	1	405098	5	NULL	NULL	0	NULL	Phasic entry 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Phasic entry of calcium in response to depolarization of giant axons of Loligo forbesi .
	manualset3
123796	2	405098	5	NULL	NULL	0	NULL	calcium 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Phasic entry of calcium in response to depolarization of giant axons of Loligo forbesi .
	manualset3
123797	3	405098	5	NULL	NULL	0	NULL	depolarization 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Phasic entry of calcium in response to depolarization of giant axons of Loligo forbesi .
	manualset3
123798	4	405098	5	NULL	NULL	0	NULL	giant axons 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Phasic entry of calcium in response to depolarization of giant axons of Loligo forbesi .
	manualset3
123799	5	405098	5	NULL	NULL	0	NULL	Loligo forbesi	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Phasic entry of calcium in response to depolarization of giant axons of Loligo forbesi .
	manualset3
123800	1	405099	5	NULL	NULL	0	NULL	Phencyclidine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Phencyclidine ( 20 mg/kg , i.p. ) , given in place of chlormethiazole , also prevented the loss of tyrosine hydroxylase .
	manualset3
123801	2	405099	5	NULL	NULL	0	NULL	20 mg/kg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Phencyclidine ( 20 mg/kg , i.p. ) , given in place of chlormethiazole , also prevented the loss of tyrosine hydroxylase .
	manualset3
123802	3	405099	5	NULL	NULL	0	NULL	place 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phencyclidine ( 20 mg/kg , i.p. ) , given in place of chlormethiazole , also prevented the loss of tyrosine hydroxylase .
	manualset3
123803	4	405099	5	NULL	NULL	0	NULL	chlormethiazole 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Phencyclidine ( 20 mg/kg , i.p. ) , given in place of chlormethiazole , also prevented the loss of tyrosine hydroxylase .
	manualset3
123804	5	405099	5	NULL	NULL	0	NULL	loss 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Phencyclidine ( 20 mg/kg , i.p. ) , given in place of chlormethiazole , also prevented the loss of tyrosine hydroxylase .
	manualset3
123805	6	405099	5	NULL	NULL	0	NULL	tyrosine hydroxylase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Phencyclidine ( 20 mg/kg , i.p. ) , given in place of chlormethiazole , also prevented the loss of tyrosine hydroxylase .
	manualset3
123806	1	405100	5	NULL	NULL	0	NULL	Phenotype 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phenotype correlated with in situ fibroblast phenotype in the tissues of origin .
	manualset3
123807	2	405100	5	NULL	NULL	0	NULL	 in situ fibroblast phenotype	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phenotype correlated with in situ fibroblast phenotype in the tissues of origin .
	manualset3
123808	3	405100	5	NULL	NULL	0	NULL	tissues 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Phenotype correlated with in situ fibroblast phenotype in the tissues of origin .
	manualset3
123809	4	405100	5	NULL	NULL	0	NULL	origin 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phenotype correlated with in situ fibroblast phenotype in the tissues of origin .
	manualset3
123810	1	405101	5	NULL	NULL	0	NULL	Phenotypic Characterization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Phenotypic Characterization of a copA Mutant of Neisseria gonorrhoeae Identifies a Link between Copper and Nitrosative Stress .
	manualset3
123811	2	405101	5	NULL	NULL	0	NULL	copA Mutant	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Phenotypic Characterization of a copA Mutant of Neisseria gonorrhoeae Identifies a Link between Copper and Nitrosative Stress .
	manualset3
123812	3	405101	5	NULL	NULL	0	NULL	Neisseria gonorrhoeae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Phenotypic Characterization of a copA Mutant of Neisseria gonorrhoeae Identifies a Link between Copper and Nitrosative Stress .
	manualset3
123813	4	405101	5	NULL	NULL	0	NULL	Link 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phenotypic Characterization of a copA Mutant of Neisseria gonorrhoeae Identifies a Link between Copper and Nitrosative Stress .
	manualset3
123814	5	405101	5	NULL	NULL	0	NULL	Copper 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Phenotypic Characterization of a copA Mutant of Neisseria gonorrhoeae Identifies a Link between Copper and Nitrosative Stress .
	manualset3
123815	6	405101	5	NULL	NULL	0	NULL	Nitrosative Stress	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Phenotypic Characterization of a copA Mutant of Neisseria gonorrhoeae Identifies a Link between Copper and Nitrosative Stress .
	manualset3
123816	1	405102	5	NULL	NULL	0	NULL	growing number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A growing number of proteins and small molecules have been identified that regulate HIF-1 activity by modulating the physical or functional interaction of PHD2 , VHL , FIH-1 , RACK1 , or HSP90 with HIF-1alpha .
	manualset3
123817	2	405102	5	NULL	NULL	0	NULL	proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A growing number of proteins and small molecules have been identified that regulate HIF-1 activity by modulating the physical or functional interaction of PHD2 , VHL , FIH-1 , RACK1 , or HSP90 with HIF-1alpha .
	manualset3
123818	3	405102	5	NULL	NULL	0	NULL	small molecules 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A growing number of proteins and small molecules have been identified that regulate HIF-1 activity by modulating the physical or functional interaction of PHD2 , VHL , FIH-1 , RACK1 , or HSP90 with HIF-1alpha .
	manualset3
123819	4	405102	5	NULL	NULL	0	NULL	HIF-1 activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A growing number of proteins and small molecules have been identified that regulate HIF-1 activity by modulating the physical or functional interaction of PHD2 , VHL , FIH-1 , RACK1 , or HSP90 with HIF-1alpha .
	manualset3
123820	5	405102	5	NULL	NULL	0	NULL	physical interaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A growing number of proteins and small molecules have been identified that regulate HIF-1 activity by modulating the physical or functional interaction of PHD2 , VHL , FIH-1 , RACK1 , or HSP90 with HIF-1alpha .
	manualset3
123821	6	405102	5	NULL	NULL	0	NULL	functional interaction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A growing number of proteins and small molecules have been identified that regulate HIF-1 activity by modulating the physical or functional interaction of PHD2 , VHL , FIH-1 , RACK1 , or HSP90 with HIF-1alpha .
	manualset3
123822	7	405102	5	NULL	NULL	0	NULL	PHD2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A growing number of proteins and small molecules have been identified that regulate HIF-1 activity by modulating the physical or functional interaction of PHD2 , VHL , FIH-1 , RACK1 , or HSP90 with HIF-1alpha .
	manualset3
123823	8	405102	5	NULL	NULL	0	NULL	VHL 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A growing number of proteins and small molecules have been identified that regulate HIF-1 activity by modulating the physical or functional interaction of PHD2 , VHL , FIH-1 , RACK1 , or HSP90 with HIF-1alpha .
	manualset3
123824	9	405102	5	NULL	NULL	0	NULL	FIH-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A growing number of proteins and small molecules have been identified that regulate HIF-1 activity by modulating the physical or functional interaction of PHD2 , VHL , FIH-1 , RACK1 , or HSP90 with HIF-1alpha .
	manualset3
123825	10	405102	5	NULL	NULL	0	NULL	RACK1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A growing number of proteins and small molecules have been identified that regulate HIF-1 activity by modulating the physical or functional interaction of PHD2 , VHL , FIH-1 , RACK1 , or HSP90 with HIF-1alpha .
	manualset3
123826	11	405102	5	NULL	NULL	0	NULL	HSP90 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A growing number of proteins and small molecules have been identified that regulate HIF-1 activity by modulating the physical or functional interaction of PHD2 , VHL , FIH-1 , RACK1 , or HSP90 with HIF-1alpha .
	manualset3
123827	12	405102	5	NULL	NULL	0	NULL	HIF-1alpha 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A growing number of proteins and small molecules have been identified that regulate HIF-1 activity by modulating the physical or functional interaction of PHD2 , VHL , FIH-1 , RACK1 , or HSP90 with HIF-1alpha .
	manualset3
123850	1	405103	5	NULL	NULL	0	NULL	Phenylalkyl 1 , 2-diamines 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Phenylalkyl 1 , 2-diamines as sigma-receptor ligands : the discovery of novel antidepressant agents .
	manualset3
123851	2	405103	5	NULL	NULL	0	NULL	sigma-receptor ligands	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Phenylalkyl 1 , 2-diamines as sigma-receptor ligands : the discovery of novel antidepressant agents .
	manualset3
123852	3	405103	5	NULL	NULL	0	NULL	discovery 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Phenylalkyl 1 , 2-diamines as sigma-receptor ligands : the discovery of novel antidepressant agents .
	manualset3
123853	4	405103	5	NULL	NULL	0	NULL	novel antidepressant agents	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Phenylalkyl 1 , 2-diamines as sigma-receptor ligands : the discovery of novel antidepressant agents .
	manualset3
123854	1	405104	5	NULL	NULL	0	NULL	Pheochromocytoma cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Pheochromocytoma cell lines derived from neurofibromatosis knockout mice express high levels of the receptor tyrosine kinase Ret , which is involved in the pathogenesis of human pheochromocytomas in hereditary multiple endocrine neoplasia syndrome type 2 ( MEN2 ) .
	manualset3
123855	2	405104	5	NULL	NULL	0	NULL	neurofibromatosis knockout mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pheochromocytoma cell lines derived from neurofibromatosis knockout mice express high levels of the receptor tyrosine kinase Ret , which is involved in the pathogenesis of human pheochromocytomas in hereditary multiple endocrine neoplasia syndrome type 2 ( MEN2 ) .
	manualset3
123856	3	405104	5	NULL	NULL	0	NULL	high levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pheochromocytoma cell lines derived from neurofibromatosis knockout mice express high levels of the receptor tyrosine kinase Ret , which is involved in the pathogenesis of human pheochromocytomas in hereditary multiple endocrine neoplasia syndrome type 2 ( MEN2 ) .
	manualset3
123857	4	405104	5	NULL	NULL	0	NULL	receptor tyrosine kinase Ret 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Pheochromocytoma cell lines derived from neurofibromatosis knockout mice express high levels of the receptor tyrosine kinase Ret , which is involved in the pathogenesis of human pheochromocytomas in hereditary multiple endocrine neoplasia syndrome type 2 ( MEN2 ) .
	manualset3
123859	5	405104	5	NULL	NULL	0	NULL	pathogenesis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pheochromocytoma cell lines derived from neurofibromatosis knockout mice express high levels of the receptor tyrosine kinase Ret , which is involved in the pathogenesis of human pheochromocytomas in hereditary multiple endocrine neoplasia syndrome type 2 ( MEN2 ) .
	manualset3
123860	6	405104	5	NULL	NULL	0	NULL	human pheochromocytomas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pheochromocytoma cell lines derived from neurofibromatosis knockout mice express high levels of the receptor tyrosine kinase Ret , which is involved in the pathogenesis of human pheochromocytomas in hereditary multiple endocrine neoplasia syndrome type 2 ( MEN2 ) .
	manualset3
123861	7	405104	5	NULL	NULL	0	NULL	hereditary multiple endocrine neoplasia syndrome type 2 ( MEN2 )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pheochromocytoma cell lines derived from neurofibromatosis knockout mice express high levels of the receptor tyrosine kinase Ret , which is involved in the pathogenesis of human pheochromocytomas in hereditary multiple endocrine neoplasia syndrome type 2 ( MEN2 ) .
	manualset3
123862	1	405105	5	NULL	NULL	0	NULL	Phosphaturic mesenchymal tumor 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphaturic mesenchymal tumor with chondromyxoid fibroma-like feature : an unusual morphological appearance .
	manualset3
123863	2	405105	5	NULL	NULL	0	NULL	chondromyxoid fibroma-like feature	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphaturic mesenchymal tumor with chondromyxoid fibroma-like feature : an unusual morphological appearance .
	manualset3
123865	3	405105	5	NULL	NULL	0	NULL	morphological appearance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphaturic mesenchymal tumor with chondromyxoid fibroma-like feature : an unusual morphological appearance .
	manualset3
123872	1	405106	5	NULL	NULL	0	NULL	Phospho enolpyruvate carboxykinase ( PEPCK )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospho enolpyruvate carboxykinase ( PEPCK ) plays an important role in gluconeogenesis and hepatic glucose production .
	manualset3
123873	2	405106	5	NULL	NULL	0	NULL	important role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospho enolpyruvate carboxykinase ( PEPCK ) plays an important role in gluconeogenesis and hepatic glucose production .
	manualset3
123874	3	405106	5	NULL	NULL	0	NULL	gluconeogenesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospho enolpyruvate carboxykinase ( PEPCK ) plays an important role in gluconeogenesis and hepatic glucose production .
	manualset3
123875	4	405106	5	NULL	NULL	0	NULL	hepatic glucose production 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospho enolpyruvate carboxykinase ( PEPCK ) plays an important role in gluconeogenesis and hepatic glucose production .
	manualset3
123877	1	405107	5	NULL	NULL	0	NULL	Phosphoenolpyruvate carboxykinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphoenolpyruvate carboxykinase from bullfrog liver mitochondria has been purified to electrophoretical and immunological homogeneity by an improved method using hydrophobic chromatography on Sepharose-hexane-GMP and affinity chromatography on phosphocellulose .
	manualset3
123878	2	405107	5	NULL	NULL	0	NULL	bullfrog liver mitochondria	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphoenolpyruvate carboxykinase from bullfrog liver mitochondria has been purified to electrophoretical and immunological homogeneity by an improved method using hydrophobic chromatography on Sepharose-hexane-GMP and affinity chromatography on phosphocellulose .
	manualset3
123879	3	405107	5	NULL	NULL	0	NULL	electrophoretical homogeneity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphoenolpyruvate carboxykinase from bullfrog liver mitochondria has been purified to electrophoretical and immunological homogeneity by an improved method using hydrophobic chromatography on Sepharose-hexane-GMP and affinity chromatography on phosphocellulose .
	manualset3
123880	4	405107	5	NULL	NULL	0	NULL	 immunological homogeneity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphoenolpyruvate carboxykinase from bullfrog liver mitochondria has been purified to electrophoretical and immunological homogeneity by an improved method using hydrophobic chromatography on Sepharose-hexane-GMP and affinity chromatography on phosphocellulose .
	manualset3
123881	5	405107	5	NULL	NULL	0	NULL	method 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphoenolpyruvate carboxykinase from bullfrog liver mitochondria has been purified to electrophoretical and immunological homogeneity by an improved method using hydrophobic chromatography on Sepharose-hexane-GMP and affinity chromatography on phosphocellulose .
	manualset3
123882	6	405107	5	NULL	NULL	0	NULL	hydrophobic chromatography 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphoenolpyruvate carboxykinase from bullfrog liver mitochondria has been purified to electrophoretical and immunological homogeneity by an improved method using hydrophobic chromatography on Sepharose-hexane-GMP and affinity chromatography on phosphocellulose .
	manualset3
123885	7	405107	5	NULL	NULL	0	NULL	Sepharose-hexane-GMP chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphoenolpyruvate carboxykinase from bullfrog liver mitochondria has been purified to electrophoretical and immunological homogeneity by an improved method using hydrophobic chromatography on Sepharose-hexane-GMP and affinity chromatography on phosphocellulose .
	manualset3
123887	8	405107	5	NULL	NULL	0	NULL	affinity chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphoenolpyruvate carboxykinase from bullfrog liver mitochondria has been purified to electrophoretical and immunological homogeneity by an improved method using hydrophobic chromatography on Sepharose-hexane-GMP and affinity chromatography on phosphocellulose .
	manualset3
123890	9	405107	5	NULL	NULL	0	NULL	phosphocellulose 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphoenolpyruvate carboxykinase from bullfrog liver mitochondria has been purified to electrophoretical and immunological homogeneity by an improved method using hydrophobic chromatography on Sepharose-hexane-GMP and affinity chromatography on phosphocellulose .
	manualset3
123891	1	405108	5	NULL	NULL	0	NULL	Phosphofructokinase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphofructokinase in Escherichia coli is such an enzyme , being inhibited by phosphoenolpyruvate ( PEP ) and activated by ADP and GDP .
	manualset3
123892	2	405108	5	NULL	NULL	0	NULL	Escherichia coli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphofructokinase in Escherichia coli is such an enzyme , being inhibited by phosphoenolpyruvate ( PEP ) and activated by ADP and GDP .
	manualset3
123893	3	405108	5	NULL	NULL	0	NULL	enzyme 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphofructokinase in Escherichia coli is such an enzyme , being inhibited by phosphoenolpyruvate ( PEP ) and activated by ADP and GDP .
	manualset3
123894	4	405108	5	NULL	NULL	0	NULL	phosphoenolpyruvate ( PEP ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphofructokinase in Escherichia coli is such an enzyme , being inhibited by phosphoenolpyruvate ( PEP ) and activated by ADP and GDP .
	manualset3
123895	5	405108	5	NULL	NULL	0	NULL	ADP 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphofructokinase in Escherichia coli is such an enzyme , being inhibited by phosphoenolpyruvate ( PEP ) and activated by ADP and GDP .
	manualset3
123896	6	405108	5	NULL	NULL	0	NULL	GDP 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphofructokinase in Escherichia coli is such an enzyme , being inhibited by phosphoenolpyruvate ( PEP ) and activated by ADP and GDP .
	manualset3
123898	1	405109	5	NULL	NULL	0	NULL	Phospholipid analyses 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospholipid analyses of plasma membrane preparations showed the presence of the same four major phospholipid groups as in the human erythrocyte , although with higher and lower amounts of phosphatidylcholine and sphingomyelin , respectively .
	manualset3
123900	2	405109	5	NULL	NULL	0	NULL	plasma membrane preparations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospholipid analyses of plasma membrane preparations showed the presence of the same four major phospholipid groups as in the human erythrocyte , although with higher and lower amounts of phosphatidylcholine and sphingomyelin , respectively .
	manualset3
123902	3	405109	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospholipid analyses of plasma membrane preparations showed the presence of the same four major phospholipid groups as in the human erythrocyte , although with higher and lower amounts of phosphatidylcholine and sphingomyelin , respectively .
	manualset3
123903	4	405109	5	NULL	NULL	0	NULL	four 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospholipid analyses of plasma membrane preparations showed the presence of the same four major phospholipid groups as in the human erythrocyte , although with higher and lower amounts of phosphatidylcholine and sphingomyelin , respectively .
	manualset3
123904	5	405109	5	NULL	NULL	0	NULL	major phospholipid groups	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospholipid analyses of plasma membrane preparations showed the presence of the same four major phospholipid groups as in the human erythrocyte , although with higher and lower amounts of phosphatidylcholine and sphingomyelin , respectively .
	manualset3
123905	6	405109	5	NULL	NULL	0	NULL	human erythrocyte	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospholipid analyses of plasma membrane preparations showed the presence of the same four major phospholipid groups as in the human erythrocyte , although with higher and lower amounts of phosphatidylcholine and sphingomyelin , respectively .
	manualset3
123906	7	405109	5	NULL	NULL	0	NULL	higher amounts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospholipid analyses of plasma membrane preparations showed the presence of the same four major phospholipid groups as in the human erythrocyte , although with higher and lower amounts of phosphatidylcholine and sphingomyelin , respectively .
	manualset3
123907	8	405109	5	NULL	NULL	0	NULL	lower amounts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospholipid analyses of plasma membrane preparations showed the presence of the same four major phospholipid groups as in the human erythrocyte , although with higher and lower amounts of phosphatidylcholine and sphingomyelin , respectively .
	manualset3
123920	9	405109	5	NULL	NULL	NULL	NULL	phosphatidylcholine 	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Phospholipid analyses of plasma membrane preparations showed the presence of the same four major phospholipid groups as in the human erythrocyte , although with higher and lower amounts of phosphatidylcholine and sphingomyelin , respectively .
	manualset3
123929	10	405109	5	NULL	NULL	NULL	NULL	sphingomyelin	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Phospholipid analyses of plasma membrane preparations showed the presence of the same four major phospholipid groups as in the human erythrocyte , although with higher and lower amounts of phosphatidylcholine and sphingomyelin , respectively .
	manualset3
123934	1	405110	5	NULL	NULL	0	NULL	CYFRA 21.1 cytosol levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( CYFRA 21.1 cytosol levels in lung adenocarcinomas .
	manualset3
123935	2	405110	5	NULL	NULL	0	NULL	lung adenocarcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( CYFRA 21.1 cytosol levels in lung adenocarcinomas .
	manualset3
123936	1	405111	5	NULL	NULL	0	NULL	guide 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A guide by collaborators in Oregon recommends putting all would-be partners ' goals on the table and lining up solid financial support before undertaking an alliance of managed care , medical school and health system .
	manualset3
123937	2	405111	5	NULL	NULL	0	NULL	collaborators 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A guide by collaborators in Oregon recommends putting all would-be partners ' goals on the table and lining up solid financial support before undertaking an alliance of managed care , medical school and health system .
	manualset3
123938	3	405111	5	NULL	NULL	0	NULL	Oregon 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A guide by collaborators in Oregon recommends putting all would-be partners ' goals on the table and lining up solid financial support before undertaking an alliance of managed care , medical school and health system .
	manualset3
123942	4	405111	5	NULL	NULL	0	NULL	would-be partners ' goals	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A guide by collaborators in Oregon recommends putting all would-be partners ' goals on the table and lining up solid financial support before undertaking an alliance of managed care , medical school and health system .
	manualset3
123943	5	405111	5	NULL	NULL	0	NULL	table 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A guide by collaborators in Oregon recommends putting all would-be partners ' goals on the table and lining up solid financial support before undertaking an alliance of managed care , medical school and health system .
	manualset3
124172	6	405111	5	NULL	NULL	0	NULL	solid financial support	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A guide by collaborators in Oregon recommends putting all would-be partners ' goals on the table and lining up solid financial support before undertaking an alliance of managed care , medical school and health system .
	manualset3
124173	7	405111	5	NULL	NULL	0	NULL	alliance 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A guide by collaborators in Oregon recommends putting all would-be partners ' goals on the table and lining up solid financial support before undertaking an alliance of managed care , medical school and health system .
	manualset3
124174	8	405111	5	NULL	NULL	0	NULL	managed care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A guide by collaborators in Oregon recommends putting all would-be partners ' goals on the table and lining up solid financial support before undertaking an alliance of managed care , medical school and health system .
	manualset3
124175	9	405111	5	NULL	NULL	0	NULL	medical school 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A guide by collaborators in Oregon recommends putting all would-be partners ' goals on the table and lining up solid financial support before undertaking an alliance of managed care , medical school and health system .
	manualset3
124176	10	405111	5	NULL	NULL	0	NULL	health system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A guide by collaborators in Oregon recommends putting all would-be partners ' goals on the table and lining up solid financial support before undertaking an alliance of managed care , medical school and health system .
	manualset3
124177	1	405112	5	NULL	NULL	0	NULL	Phospholipids 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospholipids were phosphatidylglycerol , phosphatidylethanolamine , phosphatidylinositol , diphosphatidyl glycerol , methylphosphatidylethanolamine , phosphatidylserine , phosphatidylcholine and an unidentified phospholipid .
	manualset3
124178	2	405112	5	NULL	NULL	0	NULL	phosphatidylglycerol 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospholipids were phosphatidylglycerol , phosphatidylethanolamine , phosphatidylinositol , diphosphatidyl glycerol , methylphosphatidylethanolamine , phosphatidylserine , phosphatidylcholine and an unidentified phospholipid .
	manualset3
124179	3	405112	5	NULL	NULL	0	NULL	phosphatidylethanolamine 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospholipids were phosphatidylglycerol , phosphatidylethanolamine , phosphatidylinositol , diphosphatidyl glycerol , methylphosphatidylethanolamine , phosphatidylserine , phosphatidylcholine and an unidentified phospholipid .
	manualset3
124180	4	405112	5	NULL	NULL	0	NULL	phosphatidylinositol 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospholipids were phosphatidylglycerol , phosphatidylethanolamine , phosphatidylinositol , diphosphatidyl glycerol , methylphosphatidylethanolamine , phosphatidylserine , phosphatidylcholine and an unidentified phospholipid .
	manualset3
124181	5	405112	5	NULL	NULL	0	NULL	diphosphatidyl glycerol 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospholipids were phosphatidylglycerol , phosphatidylethanolamine , phosphatidylinositol , diphosphatidyl glycerol , methylphosphatidylethanolamine , phosphatidylserine , phosphatidylcholine and an unidentified phospholipid .
	manualset3
124182	6	405112	5	NULL	NULL	0	NULL	methylphosphatidylethanolamine 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospholipids were phosphatidylglycerol , phosphatidylethanolamine , phosphatidylinositol , diphosphatidyl glycerol , methylphosphatidylethanolamine , phosphatidylserine , phosphatidylcholine and an unidentified phospholipid .
	manualset3
124183	7	405112	5	NULL	NULL	0	NULL	phosphatidylserine 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospholipids were phosphatidylglycerol , phosphatidylethanolamine , phosphatidylinositol , diphosphatidyl glycerol , methylphosphatidylethanolamine , phosphatidylserine , phosphatidylcholine and an unidentified phospholipid .
	manualset3
124184	8	405112	5	NULL	NULL	0	NULL	phosphatidylcholine 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospholipids were phosphatidylglycerol , phosphatidylethanolamine , phosphatidylinositol , diphosphatidyl glycerol , methylphosphatidylethanolamine , phosphatidylserine , phosphatidylcholine and an unidentified phospholipid .
	manualset3
124185	9	405112	5	NULL	NULL	0	NULL	unidentified phospholipid	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospholipids were phosphatidylglycerol , phosphatidylethanolamine , phosphatidylinositol , diphosphatidyl glycerol , methylphosphatidylethanolamine , phosphatidylserine , phosphatidylcholine and an unidentified phospholipid .
	manualset3
124186	1	405113	5	NULL	NULL	0	NULL	Phosphopeptide mapping 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphopeptide mapping and immunoblotting with phospho-specific antibodies confirmed that Thr598 and Ser601 are in vivo phosphorylation sites induced by Ras .
	manualset3
124187	2	405113	5	NULL	NULL	0	NULL	immunoblotting 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphopeptide mapping and immunoblotting with phospho-specific antibodies confirmed that Thr598 and Ser601 are in vivo phosphorylation sites induced by Ras .
	manualset3
124234	3	405113	5	NULL	NULL	0	NULL	phospho-specific antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphopeptide mapping and immunoblotting with phospho-specific antibodies confirmed that Thr598 and Ser601 are in vivo phosphorylation sites induced by Ras .
	manualset3
124236	4	405113	5	NULL	NULL	0	NULL	Thr598 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphopeptide mapping and immunoblotting with phospho-specific antibodies confirmed that Thr598 and Ser601 are in vivo phosphorylation sites induced by Ras .
	manualset3
124239	5	405113	5	NULL	NULL	0	NULL	Ser601 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphopeptide mapping and immunoblotting with phospho-specific antibodies confirmed that Thr598 and Ser601 are in vivo phosphorylation sites induced by Ras .
	manualset3
124240	6	405113	5	NULL	NULL	0	NULL	vivo phosphorylation sites	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphopeptide mapping and immunoblotting with phospho-specific antibodies confirmed that Thr598 and Ser601 are in vivo phosphorylation sites induced by Ras .
	manualset3
124244	7	405113	5	NULL	NULL	0	NULL	Ras 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphopeptide mapping and immunoblotting with phospho-specific antibodies confirmed that Thr598 and Ser601 are in vivo phosphorylation sites induced by Ras .
	manualset3
124340	1	405114	5	NULL	NULL	0	NULL	Phosphorylated , purified moesin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylated , purified moesin co-sediments with alpha - or beta/gamma-actin filaments in cationic , but not in anionic , nonionic , or amphoteric detergents .
	manualset3
124341	2	405114	5	NULL	NULL	0	NULL	alpha - or beta/gamma-actin filaments	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylated , purified moesin co-sediments with alpha - or beta/gamma-actin filaments in cationic , but not in anionic , nonionic , or amphoteric detergents .
	manualset3
124342	3	405114	5	NULL	NULL	0	NULL	cationic detergents 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylated , purified moesin co-sediments with alpha - or beta/gamma-actin filaments in cationic , but not in anionic , nonionic , or amphoteric detergents .
	manualset3
124343	4	405114	5	NULL	NULL	0	NULL	anionic detergents 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylated , purified moesin co-sediments with alpha - or beta/gamma-actin filaments in cationic , but not in anionic , nonionic , or amphoteric detergents .
	manualset3
124344	5	405114	5	NULL	NULL	0	NULL	nonionic detergents 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylated , purified moesin co-sediments with alpha - or beta/gamma-actin filaments in cationic , but not in anionic , nonionic , or amphoteric detergents .
	manualset3
124345	6	405114	5	NULL	NULL	0	NULL	amphoteric detergents 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylated , purified moesin co-sediments with alpha - or beta/gamma-actin filaments in cationic , but not in anionic , nonionic , or amphoteric detergents .
	manualset3
124346	1	405115	5	NULL	NULL	0	NULL	Phosphorylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation in LC2 did not modulate the actin-myosin and actin-HMM interactions over a wide range of KCl concentrations from 30 to 150 mM without regulatory proteins .
	manualset3
124347	2	405115	5	NULL	NULL	0	NULL	LC2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation in LC2 did not modulate the actin-myosin and actin-HMM interactions over a wide range of KCl concentrations from 30 to 150 mM without regulatory proteins .
	manualset3
124348	3	405115	5	NULL	NULL	0	NULL	actin-myosin interactions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation in LC2 did not modulate the actin-myosin and actin-HMM interactions over a wide range of KCl concentrations from 30 to 150 mM without regulatory proteins .
	manualset3
124349	4	405115	5	NULL	NULL	0	NULL	actin-HMM interactions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation in LC2 did not modulate the actin-myosin and actin-HMM interactions over a wide range of KCl concentrations from 30 to 150 mM without regulatory proteins .
	manualset3
124350	5	405115	5	NULL	NULL	0	NULL	KCl concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation in LC2 did not modulate the actin-myosin and actin-HMM interactions over a wide range of KCl concentrations from 30 to 150 mM without regulatory proteins .
	manualset3
124351	6	405115	5	NULL	NULL	0	NULL	30 to 150 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation in LC2 did not modulate the actin-myosin and actin-HMM interactions over a wide range of KCl concentrations from 30 to 150 mM without regulatory proteins .
	manualset3
124352	7	405115	5	NULL	NULL	0	NULL	regulatory proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation in LC2 did not modulate the actin-myosin and actin-HMM interactions over a wide range of KCl concentrations from 30 to 150 mM without regulatory proteins .
	manualset3
124353	1	405116	5	NULL	NULL	0	NULL	Phosphorylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation of Elk-1 in vitro by partially purified p42/p44 MAP kinase induces a similar reduction in ternary complex mobility but has little effect on the efficiency of its formation .
	manualset3
124354	2	405116	5	NULL	NULL	0	NULL	Elk-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation of Elk-1 in vitro by partially purified p42/p44 MAP kinase induces a similar reduction in ternary complex mobility but has little effect on the efficiency of its formation .
	manualset3
124355	3	405116	5	NULL	NULL	0	NULL	partially purified p42/p44 MAP kinase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation of Elk-1 in vitro by partially purified p42/p44 MAP kinase induces a similar reduction in ternary complex mobility but has little effect on the efficiency of its formation .
	manualset3
124356	4	405116	5	NULL	NULL	0	NULL	reduction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation of Elk-1 in vitro by partially purified p42/p44 MAP kinase induces a similar reduction in ternary complex mobility but has little effect on the efficiency of its formation .
	manualset3
124357	5	405116	5	NULL	NULL	0	NULL	ternary complex mobility	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation of Elk-1 in vitro by partially purified p42/p44 MAP kinase induces a similar reduction in ternary complex mobility but has little effect on the efficiency of its formation .
	manualset3
124358	6	405116	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation of Elk-1 in vitro by partially purified p42/p44 MAP kinase induces a similar reduction in ternary complex mobility but has little effect on the efficiency of its formation .
	manualset3
124359	7	405116	5	NULL	NULL	0	NULL	efficiency 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation of Elk-1 in vitro by partially purified p42/p44 MAP kinase induces a similar reduction in ternary complex mobility but has little effect on the efficiency of its formation .
	manualset3
124360	8	405116	5	NULL	NULL	0	NULL	formation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation of Elk-1 in vitro by partially purified p42/p44 MAP kinase induces a similar reduction in ternary complex mobility but has little effect on the efficiency of its formation .
	manualset3
124361	1	405117	5	NULL	NULL	0	NULL	Phosphorylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation of eukaryotic translation initiation factor 4E is increased in Src-transformed cell lines .
	manualset3
124362	2	405117	5	NULL	NULL	0	NULL	eukaryotic translation initiation factor 4E	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation of eukaryotic translation initiation factor 4E is increased in Src-transformed cell lines .
	manualset3
124363	3	405117	5	NULL	NULL	0	NULL	Src-transformed cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation of eukaryotic translation initiation factor 4E is increased in Src-transformed cell lines .
	manualset3
124364	1	405118	5	NULL	NULL	0	NULL	Phosphorylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation of serine 28 by PKR promotes mitochondrial localization of B56alpha , because wild-type but not mutant S28A B56alpha promoted mitochondrial PP2A activity .
	manualset3
124365	2	405118	5	NULL	NULL	0	NULL	serine 28	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation of serine 28 by PKR promotes mitochondrial localization of B56alpha , because wild-type but not mutant S28A B56alpha promoted mitochondrial PP2A activity .
	manualset3
124366	3	405118	5	NULL	NULL	0	NULL	PKR 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation of serine 28 by PKR promotes mitochondrial localization of B56alpha , because wild-type but not mutant S28A B56alpha promoted mitochondrial PP2A activity .
	manualset3
124367	4	405118	5	NULL	NULL	0	NULL	mitochondrial localization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation of serine 28 by PKR promotes mitochondrial localization of B56alpha , because wild-type but not mutant S28A B56alpha promoted mitochondrial PP2A activity .
	manualset3
124368	5	405118	5	NULL	NULL	0	NULL	B56alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation of serine 28 by PKR promotes mitochondrial localization of B56alpha , because wild-type but not mutant S28A B56alpha promoted mitochondrial PP2A activity .
	manualset3
124369	6	405118	5	NULL	NULL	0	NULL	wild-type B56alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation of serine 28 by PKR promotes mitochondrial localization of B56alpha , because wild-type but not mutant S28A B56alpha promoted mitochondrial PP2A activity .
	manualset3
124370	7	405118	5	NULL	NULL	0	NULL	mutant S28A B56alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation of serine 28 by PKR promotes mitochondrial localization of B56alpha , because wild-type but not mutant S28A B56alpha promoted mitochondrial PP2A activity .
	manualset3
124371	8	405118	5	NULL	NULL	0	NULL	mitochondrial PP2A activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation of serine 28 by PKR promotes mitochondrial localization of B56alpha , because wild-type but not mutant S28A B56alpha promoted mitochondrial PP2A activity .
	manualset3
124372	1	405119	5	NULL	NULL	0	NULL	Photoluminescence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Photo - and electroluminescence in thin films of covalently bonded azomethin-zinc/SiO2 hybrid materials .
	manualset3
124373	2	405119	5	NULL	NULL	0	NULL	electroluminescence 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Photo - and electroluminescence in thin films of covalently bonded azomethin-zinc/SiO2 hybrid materials .
	manualset3
124374	3	405119	5	NULL	NULL	NULL	NULL	thin films of covalently bonded azomethin-zinc/SiO2 hybrid materials	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Photo - and electroluminescence in thin films of covalently bonded azomethin-zinc/SiO2 hybrid materials .
	manualset3
124375	1	405120	5	NULL	NULL	0	NULL	Photochemical reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Photochemical reaction of ( 125 ) I-labelled ( 4-azidobenzoyl ) - N-hydroxysuccinimide - ( d-Lys ( 6 ) ) - GnRH-II ( 10 ( -9 ) M ) with cell membrane preparations of human endometrial and ovarian cancer cells yielded a band at approximately 43 kDa .
	manualset3
124376	2	405120	5	NULL	NULL	0	NULL	( 125 ) I-labelled ( 4-azidobenzoyl ) - N-hydroxysuccinimide - ( d-Lys ( 6 ) ) - GnRH-II ( 10 ( -9 ) M ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Photochemical reaction of ( 125 ) I-labelled ( 4-azidobenzoyl ) - N-hydroxysuccinimide - ( d-Lys ( 6 ) ) - GnRH-II ( 10 ( -9 ) M ) with cell membrane preparations of human endometrial and ovarian cancer cells yielded a band at approximately 43 kDa .
	manualset3
124377	3	405120	5	NULL	NULL	0	NULL	cell membrane preparations	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Photochemical reaction of ( 125 ) I-labelled ( 4-azidobenzoyl ) - N-hydroxysuccinimide - ( d-Lys ( 6 ) ) - GnRH-II ( 10 ( -9 ) M ) with cell membrane preparations of human endometrial and ovarian cancer cells yielded a band at approximately 43 kDa .
	manualset3
124378	4	405120	5	NULL	NULL	0	NULL	human endometrial cancer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Photochemical reaction of ( 125 ) I-labelled ( 4-azidobenzoyl ) - N-hydroxysuccinimide - ( d-Lys ( 6 ) ) - GnRH-II ( 10 ( -9 ) M ) with cell membrane preparations of human endometrial and ovarian cancer cells yielded a band at approximately 43 kDa .
	manualset3
124379	5	405120	5	NULL	NULL	0	NULL	human ovarian cancer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Photochemical reaction of ( 125 ) I-labelled ( 4-azidobenzoyl ) - N-hydroxysuccinimide - ( d-Lys ( 6 ) ) - GnRH-II ( 10 ( -9 ) M ) with cell membrane preparations of human endometrial and ovarian cancer cells yielded a band at approximately 43 kDa .
	manualset3
124380	6	405120	5	NULL	NULL	0	NULL	band 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Photochemical reaction of ( 125 ) I-labelled ( 4-azidobenzoyl ) - N-hydroxysuccinimide - ( d-Lys ( 6 ) ) - GnRH-II ( 10 ( -9 ) M ) with cell membrane preparations of human endometrial and ovarian cancer cells yielded a band at approximately 43 kDa .
	manualset3
124381	7	405120	5	NULL	NULL	0	NULL	43 kDa	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Photochemical reaction of ( 125 ) I-labelled ( 4-azidobenzoyl ) - N-hydroxysuccinimide - ( d-Lys ( 6 ) ) - GnRH-II ( 10 ( -9 ) M ) with cell membrane preparations of human endometrial and ovarian cancer cells yielded a band at approximately 43 kDa .
	manualset3
124382	1	405121	5	NULL	NULL	0	NULL	Photodynamic effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Photodynamic effect of dye on frog muscle fiber using microelectrodes .
	manualset3
124383	2	405121	5	NULL	NULL	0	NULL	dye 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Photodynamic effect of dye on frog muscle fiber using microelectrodes .
	manualset3
124384	3	405121	5	NULL	NULL	0	NULL	frog muscle fiber	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Photodynamic effect of dye on frog muscle fiber using microelectrodes .
	manualset3
124385	4	405121	5	NULL	NULL	0	NULL	microelectrodes 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Photodynamic effect of dye on frog muscle fiber using microelectrodes .
	manualset3
124386	1	405122	5	NULL	NULL	0	NULL	Photodynamic therapy ( PDT )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Photodynamic therapy ( PDT ) involves the activation of a photosensitizing drug , which preferentially localizes to diseased skin , by irradiation with light to cause selective cytotoxic damage .
	manualset3
124387	2	405122	5	NULL	NULL	0	NULL	activation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Photodynamic therapy ( PDT ) involves the activation of a photosensitizing drug , which preferentially localizes to diseased skin , by irradiation with light to cause selective cytotoxic damage .
	manualset3
124388	3	405122	5	NULL	NULL	0	NULL	photosensitizing drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Photodynamic therapy ( PDT ) involves the activation of a photosensitizing drug , which preferentially localizes to diseased skin , by irradiation with light to cause selective cytotoxic damage .
	manualset3
124389	4	405122	5	NULL	NULL	0	NULL	diseased skin 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Photodynamic therapy ( PDT ) involves the activation of a photosensitizing drug , which preferentially localizes to diseased skin , by irradiation with light to cause selective cytotoxic damage .
	manualset3
124390	5	405122	5	NULL	NULL	0	NULL	irradiation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Photodynamic therapy ( PDT ) involves the activation of a photosensitizing drug , which preferentially localizes to diseased skin , by irradiation with light to cause selective cytotoxic damage .
	manualset3
124391	6	405122	5	NULL	NULL	0	NULL	light 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Photodynamic therapy ( PDT ) involves the activation of a photosensitizing drug , which preferentially localizes to diseased skin , by irradiation with light to cause selective cytotoxic damage .
	manualset3
124392	7	405122	5	NULL	NULL	0	NULL	selective cytotoxic damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Photodynamic therapy ( PDT ) involves the activation of a photosensitizing drug , which preferentially localizes to diseased skin , by irradiation with light to cause selective cytotoxic damage .
	manualset3
124393	1	405123	5	NULL	NULL	0	NULL	Photodynamic therapy ( PDT )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Photodynamic therapy ( PDT ) is a photochemotherapeutic process that is used for the treatment of cancer .
	manualset3
124394	2	405123	5	NULL	NULL	0	NULL	photochemotherapeutic process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Photodynamic therapy ( PDT ) is a photochemotherapeutic process that is used for the treatment of cancer .
	manualset3
124395	3	405123	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Photodynamic therapy ( PDT ) is a photochemotherapeutic process that is used for the treatment of cancer .
	manualset3
124396	4	405123	5	NULL	NULL	0	NULL	cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Photodynamic therapy ( PDT ) is a photochemotherapeutic process that is used for the treatment of cancer .
	manualset3
124397	1	405124	5	NULL	NULL	0	NULL	Photodynamic therapy ( PDT )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Photodynamic therapy ( PDT ) is clinically approved for the treatment of several types of cancer as well as age-related macular degeneration , the leading cause of blindness in the elderly .
	manualset3
124398	2	405124	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Photodynamic therapy ( PDT ) is clinically approved for the treatment of several types of cancer as well as age-related macular degeneration , the leading cause of blindness in the elderly .
	manualset3
124399	3	405124	5	NULL	NULL	0	NULL	several types	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Photodynamic therapy ( PDT ) is clinically approved for the treatment of several types of cancer as well as age-related macular degeneration , the leading cause of blindness in the elderly .
	manualset3
124400	4	405124	5	NULL	NULL	0	NULL	cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Photodynamic therapy ( PDT ) is clinically approved for the treatment of several types of cancer as well as age-related macular degeneration , the leading cause of blindness in the elderly .
	manualset3
124401	5	405124	5	NULL	NULL	0	NULL	age-related macular degeneration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Photodynamic therapy ( PDT ) is clinically approved for the treatment of several types of cancer as well as age-related macular degeneration , the leading cause of blindness in the elderly .
	manualset3
124402	6	405124	5	NULL	NULL	0	NULL	leading cause	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Photodynamic therapy ( PDT ) is clinically approved for the treatment of several types of cancer as well as age-related macular degeneration , the leading cause of blindness in the elderly .
	manualset3
124403	7	405124	5	NULL	NULL	0	NULL	blindness 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Photodynamic therapy ( PDT ) is clinically approved for the treatment of several types of cancer as well as age-related macular degeneration , the leading cause of blindness in the elderly .
	manualset3
124404	8	405124	5	NULL	NULL	0	NULL	elderly 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Photodynamic therapy ( PDT ) is clinically approved for the treatment of several types of cancer as well as age-related macular degeneration , the leading cause of blindness in the elderly .
	manualset3
124405	1	405125	5	NULL	NULL	0	NULL	Photogeneration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Photogeneration of superoxide and decarboxylated peptide radicals by carboquone , mitomycin C and streptonigrin .
	manualset3
124406	2	405125	5	NULL	NULL	0	NULL	superoxide 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Photogeneration of superoxide and decarboxylated peptide radicals by carboquone , mitomycin C and streptonigrin .
	manualset3
124407	3	405125	5	NULL	NULL	0	NULL	decarboxylated peptide radicals	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Photogeneration of superoxide and decarboxylated peptide radicals by carboquone , mitomycin C and streptonigrin .
	manualset3
124408	4	405125	5	NULL	NULL	0	NULL	carboquone 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Photogeneration of superoxide and decarboxylated peptide radicals by carboquone , mitomycin C and streptonigrin .
	manualset3
124409	5	405125	5	NULL	NULL	0	NULL	mitomycin C	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Photogeneration of superoxide and decarboxylated peptide radicals by carboquone , mitomycin C and streptonigrin .
	manualset3
124410	6	405125	5	NULL	NULL	0	NULL	streptonigrin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Photogeneration of superoxide and decarboxylated peptide radicals by carboquone , mitomycin C and streptonigrin .
	manualset3
124411	1	405126	5	NULL	NULL	0	NULL	Photoincorporation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Photoincorporation of ( beta-32P ) 5-N3UDP-GlcA into bovine liver UDP-Glc dehydrogenase ( EC 1.1.1.22 ) was saturable with an apparent Kd of 12.5 microM , and was inhibited by the known active-site effectors UDP-GlcA , UDP-Glc , and UDP-xylose .
	manualset3
124412	2	405126	5	NULL	NULL	0	NULL	( beta-32P ) 5-N3UDP-GlcA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Photoincorporation of ( beta-32P ) 5-N3UDP-GlcA into bovine liver UDP-Glc dehydrogenase ( EC 1.1.1.22 ) was saturable with an apparent Kd of 12.5 microM , and was inhibited by the known active-site effectors UDP-GlcA , UDP-Glc , and UDP-xylose .
	manualset3
124413	3	405126	5	NULL	NULL	0	NULL	bovine liver UDP-Glc dehydrogenase ( EC 1.1.1.22 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Photoincorporation of ( beta-32P ) 5-N3UDP-GlcA into bovine liver UDP-Glc dehydrogenase ( EC 1.1.1.22 ) was saturable with an apparent Kd of 12.5 microM , and was inhibited by the known active-site effectors UDP-GlcA , UDP-Glc , and UDP-xylose .
	manualset3
124414	4	405126	5	NULL	NULL	0	NULL	Kd	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Photoincorporation of ( beta-32P ) 5-N3UDP-GlcA into bovine liver UDP-Glc dehydrogenase ( EC 1.1.1.22 ) was saturable with an apparent Kd of 12.5 microM , and was inhibited by the known active-site effectors UDP-GlcA , UDP-Glc , and UDP-xylose .
	manualset3
124415	5	405126	5	NULL	NULL	0	NULL	12.5 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Photoincorporation of ( beta-32P ) 5-N3UDP-GlcA into bovine liver UDP-Glc dehydrogenase ( EC 1.1.1.22 ) was saturable with an apparent Kd of 12.5 microM , and was inhibited by the known active-site effectors UDP-GlcA , UDP-Glc , and UDP-xylose .
	manualset3
124416	6	405126	5	NULL	NULL	0	NULL	active-site effectors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Photoincorporation of ( beta-32P ) 5-N3UDP-GlcA into bovine liver UDP-Glc dehydrogenase ( EC 1.1.1.22 ) was saturable with an apparent Kd of 12.5 microM , and was inhibited by the known active-site effectors UDP-GlcA , UDP-Glc , and UDP-xylose .
	manualset3
124417	7	405126	5	NULL	NULL	0	NULL	UDP-GlcA	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Photoincorporation of ( beta-32P ) 5-N3UDP-GlcA into bovine liver UDP-Glc dehydrogenase ( EC 1.1.1.22 ) was saturable with an apparent Kd of 12.5 microM , and was inhibited by the known active-site effectors UDP-GlcA , UDP-Glc , and UDP-xylose .
	manualset3
124418	8	405126	5	NULL	NULL	0	NULL	UDP-Glc	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Photoincorporation of ( beta-32P ) 5-N3UDP-GlcA into bovine liver UDP-Glc dehydrogenase ( EC 1.1.1.22 ) was saturable with an apparent Kd of 12.5 microM , and was inhibited by the known active-site effectors UDP-GlcA , UDP-Glc , and UDP-xylose .
	manualset3
124419	9	405126	5	NULL	NULL	0	NULL	UDP-xylose	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Photoincorporation of ( beta-32P ) 5-N3UDP-GlcA into bovine liver UDP-Glc dehydrogenase ( EC 1.1.1.22 ) was saturable with an apparent Kd of 12.5 microM , and was inhibited by the known active-site effectors UDP-GlcA , UDP-Glc , and UDP-xylose .
	manualset3
124420	1	405127	5	NULL	NULL	0	NULL	Photoirradiation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Photoirradiation of BDH plus or minus NAD in the absence or presence of ( arylazido ) - beta-alanine caused little or no inhibition .
	manualset3
124421	2	405127	5	NULL	NULL	0	NULL	BDH plus or minus NAD	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Photoirradiation of BDH plus or minus NAD in the absence or presence of ( arylazido ) - beta-alanine caused little or no inhibition .
	manualset3
124422	3	405127	5	NULL	NULL	0	NULL	absence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Photoirradiation of BDH plus or minus NAD in the absence or presence of ( arylazido ) - beta-alanine caused little or no inhibition .
	manualset3
124423	4	405127	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Photoirradiation of BDH plus or minus NAD in the absence or presence of ( arylazido ) - beta-alanine caused little or no inhibition .
	manualset3
124424	5	405127	5	NULL	NULL	0	NULL	( arylazido ) - beta-alanine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Photoirradiation of BDH plus or minus NAD in the absence or presence of ( arylazido ) - beta-alanine caused little or no inhibition .
	manualset3
124425	6	405127	5	NULL	NULL	0	NULL	inhibition 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Photoirradiation of BDH plus or minus NAD in the absence or presence of ( arylazido ) - beta-alanine caused little or no inhibition .
	manualset3
124426	1	405128	5	NULL	NULL	0	NULL	Photolysis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Photolysis of the glucose analog in the presence of the particulate pellet derived from homogenized adipocytes resulted in the incorporation of the radioactive label into most of the membrane proteins .
	manualset3
124427	2	405128	5	NULL	NULL	0	NULL	glucose analog	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Photolysis of the glucose analog in the presence of the particulate pellet derived from homogenized adipocytes resulted in the incorporation of the radioactive label into most of the membrane proteins .
	manualset3
124428	3	405128	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Photolysis of the glucose analog in the presence of the particulate pellet derived from homogenized adipocytes resulted in the incorporation of the radioactive label into most of the membrane proteins .
	manualset3
124429	4	405128	5	NULL	NULL	0	NULL	particulate pellet 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Photolysis of the glucose analog in the presence of the particulate pellet derived from homogenized adipocytes resulted in the incorporation of the radioactive label into most of the membrane proteins .
	manualset3
124430	5	405128	5	NULL	NULL	0	NULL	homogenized adipocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Photolysis of the glucose analog in the presence of the particulate pellet derived from homogenized adipocytes resulted in the incorporation of the radioactive label into most of the membrane proteins .
	manualset3
124431	6	405128	5	NULL	NULL	0	NULL	incorporation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Photolysis of the glucose analog in the presence of the particulate pellet derived from homogenized adipocytes resulted in the incorporation of the radioactive label into most of the membrane proteins .
	manualset3
124432	7	405128	5	NULL	NULL	0	NULL	radioactive label	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Photolysis of the glucose analog in the presence of the particulate pellet derived from homogenized adipocytes resulted in the incorporation of the radioactive label into most of the membrane proteins .
	manualset3
124433	8	405128	5	NULL	NULL	0	NULL	membrane proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Photolysis of the glucose analog in the presence of the particulate pellet derived from homogenized adipocytes resulted in the incorporation of the radioactive label into most of the membrane proteins .
	manualset3
124434	1	405129	5	NULL	NULL	0	NULL	health education component	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A health education component was developed as an integral part of program inputs during the initial conceptual phase of the project .
	manualset3
124435	2	405129	5	NULL	NULL	0	NULL	integral part 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A health education component was developed as an integral part of program inputs during the initial conceptual phase of the project .
	manualset3
124436	3	405129	5	NULL	NULL	0	NULL	program 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A health education component was developed as an integral part of program inputs during the initial conceptual phase of the project .
	manualset3
124437	4	405129	5	NULL	NULL	0	NULL	initial conceptual phase	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A health education component was developed as an integral part of program inputs during the initial conceptual phase of the project .
	manualset3
124438	5	405129	5	NULL	NULL	0	NULL	project 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A health education component was developed as an integral part of program inputs during the initial conceptual phase of the project .
	manualset3
124439	1	405130	5	NULL	NULL	0	NULL	Phototherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Phototherapy was effective in decreasing bilirubin levels in both groups , but the response was greater in the double phototherapy group ; the duration of exposure to phototherapy was significantly shorter ( 31.2 + / - 8.5 vs. 38.98 + / - 14.7 h , p & lt ; 0.05 ) , and the overall bilirubin decline rate as mumol/l/h and per cent/h was significantly greater in the double phototherapy group ( 4.1 + / - 1.37 vs. 3.3 + / - 0.86 mumol/l/h , and 1.29 + / - 0.38 vs. 1.02 + / - 0.44 per cent/h , p & lt ; 0.05 ) .
	manualset3
124440	2	405130	5	NULL	NULL	0	NULL	bilirubin levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phototherapy was effective in decreasing bilirubin levels in both groups , but the response was greater in the double phototherapy group ; the duration of exposure to phototherapy was significantly shorter ( 31.2 + / - 8.5 vs. 38.98 + / - 14.7 h , p & lt ; 0.05 ) , and the overall bilirubin decline rate as mumol/l/h and per cent/h was significantly greater in the double phototherapy group ( 4.1 + / - 1.37 vs. 3.3 + / - 0.86 mumol/l/h , and 1.29 + / - 0.38 vs. 1.02 + / - 0.44 per cent/h , p & lt ; 0.05 ) .
	manualset3
124441	3	405130	5	NULL	NULL	NULL	NULL	both groups 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Phototherapy was effective in decreasing bilirubin levels in both groups , but the response was greater in the double phototherapy group ; the duration of exposure to phototherapy was significantly shorter ( 31.2 + / - 8.5 vs. 38.98 + / - 14.7 h , p & lt ; 0.05 ) , and the overall bilirubin decline rate as mumol/l/h and per cent/h was significantly greater in the double phototherapy group ( 4.1 + / - 1.37 vs. 3.3 + / - 0.86 mumol/l/h , and 1.29 + / - 0.38 vs. 1.02 + / - 0.44 per cent/h , p & lt ; 0.05 ) .
	manualset3
124442	4	405130	5	NULL	NULL	0	NULL	response 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Phototherapy was effective in decreasing bilirubin levels in both groups , but the response was greater in the double phototherapy group ; the duration of exposure to phototherapy was significantly shorter ( 31.2 + / - 8.5 vs. 38.98 + / - 14.7 h , p & lt ; 0.05 ) , and the overall bilirubin decline rate as mumol/l/h and per cent/h was significantly greater in the double phototherapy group ( 4.1 + / - 1.37 vs. 3.3 + / - 0.86 mumol/l/h , and 1.29 + / - 0.38 vs. 1.02 + / - 0.44 per cent/h , p & lt ; 0.05 ) .
	manualset3
124443	5	405130	5	NULL	NULL	0	NULL	double phototherapy group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Phototherapy was effective in decreasing bilirubin levels in both groups , but the response was greater in the double phototherapy group ; the duration of exposure to phototherapy was significantly shorter ( 31.2 + / - 8.5 vs. 38.98 + / - 14.7 h , p & lt ; 0.05 ) , and the overall bilirubin decline rate as mumol/l/h and per cent/h was significantly greater in the double phototherapy group ( 4.1 + / - 1.37 vs. 3.3 + / - 0.86 mumol/l/h , and 1.29 + / - 0.38 vs. 1.02 + / - 0.44 per cent/h , p & lt ; 0.05 ) .
	manualset3
124444	6	405130	5	NULL	NULL	0	NULL	duration 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Phototherapy was effective in decreasing bilirubin levels in both groups , but the response was greater in the double phototherapy group ; the duration of exposure to phototherapy was significantly shorter ( 31.2 + / - 8.5 vs. 38.98 + / - 14.7 h , p & lt ; 0.05 ) , and the overall bilirubin decline rate as mumol/l/h and per cent/h was significantly greater in the double phototherapy group ( 4.1 + / - 1.37 vs. 3.3 + / - 0.86 mumol/l/h , and 1.29 + / - 0.38 vs. 1.02 + / - 0.44 per cent/h , p & lt ; 0.05 ) .
	manualset3
124445	7	405130	5	NULL	NULL	0	NULL	exposure 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phototherapy was effective in decreasing bilirubin levels in both groups , but the response was greater in the double phototherapy group ; the duration of exposure to phototherapy was significantly shorter ( 31.2 + / - 8.5 vs. 38.98 + / - 14.7 h , p & lt ; 0.05 ) , and the overall bilirubin decline rate as mumol/l/h and per cent/h was significantly greater in the double phototherapy group ( 4.1 + / - 1.37 vs. 3.3 + / - 0.86 mumol/l/h , and 1.29 + / - 0.38 vs. 1.02 + / - 0.44 per cent/h , p & lt ; 0.05 ) .
	manualset3
124446	8	405130	5	NULL	NULL	0	NULL	phototherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Phototherapy was effective in decreasing bilirubin levels in both groups , but the response was greater in the double phototherapy group ; the duration of exposure to phototherapy was significantly shorter ( 31.2 + / - 8.5 vs. 38.98 + / - 14.7 h , p & lt ; 0.05 ) , and the overall bilirubin decline rate as mumol/l/h and per cent/h was significantly greater in the double phototherapy group ( 4.1 + / - 1.37 vs. 3.3 + / - 0.86 mumol/l/h , and 1.29 + / - 0.38 vs. 1.02 + / - 0.44 per cent/h , p & lt ; 0.05 ) .
	manualset3
124447	9	405130	5	NULL	NULL	0	NULL	31.2 + / - 8.5 vs. 38.98 + / - 14.7 h , p & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Phototherapy was effective in decreasing bilirubin levels in both groups , but the response was greater in the double phototherapy group ; the duration of exposure to phototherapy was significantly shorter ( 31.2 + / - 8.5 vs. 38.98 + / - 14.7 h , p & lt ; 0.05 ) , and the overall bilirubin decline rate as mumol/l/h and per cent/h was significantly greater in the double phototherapy group ( 4.1 + / - 1.37 vs. 3.3 + / - 0.86 mumol/l/h , and 1.29 + / - 0.38 vs. 1.02 + / - 0.44 per cent/h , p & lt ; 0.05 ) .
	manualset3
124448	10	405130	5	NULL	NULL	0	NULL	bilirubin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Phototherapy was effective in decreasing bilirubin levels in both groups , but the response was greater in the double phototherapy group ; the duration of exposure to phototherapy was significantly shorter ( 31.2 + / - 8.5 vs. 38.98 + / - 14.7 h , p & lt ; 0.05 ) , and the overall bilirubin decline rate as mumol/l/h and per cent/h was significantly greater in the double phototherapy group ( 4.1 + / - 1.37 vs. 3.3 + / - 0.86 mumol/l/h , and 1.29 + / - 0.38 vs. 1.02 + / - 0.44 per cent/h , p & lt ; 0.05 ) .
	manualset3
124449	11	405130	5	NULL	NULL	0	NULL	decline rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phototherapy was effective in decreasing bilirubin levels in both groups , but the response was greater in the double phototherapy group ; the duration of exposure to phototherapy was significantly shorter ( 31.2 + / - 8.5 vs. 38.98 + / - 14.7 h , p & lt ; 0.05 ) , and the overall bilirubin decline rate as mumol/l/h and per cent/h was significantly greater in the double phototherapy group ( 4.1 + / - 1.37 vs. 3.3 + / - 0.86 mumol/l/h , and 1.29 + / - 0.38 vs. 1.02 + / - 0.44 per cent/h , p & lt ; 0.05 ) .
	manualset3
124450	12	405130	5	NULL	NULL	0	NULL	 mumol/l/h	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Phototherapy was effective in decreasing bilirubin levels in both groups , but the response was greater in the double phototherapy group ; the duration of exposure to phototherapy was significantly shorter ( 31.2 + / - 8.5 vs. 38.98 + / - 14.7 h , p & lt ; 0.05 ) , and the overall bilirubin decline rate as mumol/l/h and per cent/h was significantly greater in the double phototherapy group ( 4.1 + / - 1.37 vs. 3.3 + / - 0.86 mumol/l/h , and 1.29 + / - 0.38 vs. 1.02 + / - 0.44 per cent/h , p & lt ; 0.05 ) .
	manualset3
124451	13	405130	5	NULL	NULL	0	NULL	per cent/h 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Phototherapy was effective in decreasing bilirubin levels in both groups , but the response was greater in the double phototherapy group ; the duration of exposure to phototherapy was significantly shorter ( 31.2 + / - 8.5 vs. 38.98 + / - 14.7 h , p & lt ; 0.05 ) , and the overall bilirubin decline rate as mumol/l/h and per cent/h was significantly greater in the double phototherapy group ( 4.1 + / - 1.37 vs. 3.3 + / - 0.86 mumol/l/h , and 1.29 + / - 0.38 vs. 1.02 + / - 0.44 per cent/h , p & lt ; 0.05 ) .
	manualset3
124452	14	405130	5	NULL	NULL	0	NULL	double phototherapy group 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Phototherapy was effective in decreasing bilirubin levels in both groups , but the response was greater in the double phototherapy group ; the duration of exposure to phototherapy was significantly shorter ( 31.2 + / - 8.5 vs. 38.98 + / - 14.7 h , p & lt ; 0.05 ) , and the overall bilirubin decline rate as mumol/l/h and per cent/h was significantly greater in the double phototherapy group ( 4.1 + / - 1.37 vs. 3.3 + / - 0.86 mumol/l/h , and 1.29 + / - 0.38 vs. 1.02 + / - 0.44 per cent/h , p & lt ; 0.05 ) .
	manualset3
124453	15	405130	5	NULL	NULL	0	NULL	 4.1 + / - 1.37 vs. 3.3 + / - 0.86 mumol/l/h , and 1.29 + / - 0.38 vs. 1.02 + / - 0.44 per cent/h , p & lt ; 0.05 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Phototherapy was effective in decreasing bilirubin levels in both groups , but the response was greater in the double phototherapy group ; the duration of exposure to phototherapy was significantly shorter ( 31.2 + / - 8.5 vs. 38.98 + / - 14.7 h , p & lt ; 0.05 ) , and the overall bilirubin decline rate as mumol/l/h and per cent/h was significantly greater in the double phototherapy group ( 4.1 + / - 1.37 vs. 3.3 + / - 0.86 mumol/l/h , and 1.29 + / - 0.38 vs. 1.02 + / - 0.44 per cent/h , p & lt ; 0.05 ) .
	manualset3
124736	1	405131	5	NULL	NULL	0	NULL	Phylogenetic analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analyses of the catalytic domains of the putative RTKs showed that the sponge polypeptides must be grouped with the InsRs .
	manualset3
124737	2	405131	5	NULL	NULL	0	NULL	catalytic domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analyses of the catalytic domains of the putative RTKs showed that the sponge polypeptides must be grouped with the InsRs .
	manualset3
124738	3	405131	5	NULL	NULL	0	NULL	putative RTKs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analyses of the catalytic domains of the putative RTKs showed that the sponge polypeptides must be grouped with the InsRs .
	manualset3
124739	4	405131	5	NULL	NULL	0	NULL	sponge polypeptide	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analyses of the catalytic domains of the putative RTKs showed that the sponge polypeptides must be grouped with the InsRs .
	manualset3
124740	5	405131	5	NULL	NULL	0	NULL	InsRs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analyses of the catalytic domains of the putative RTKs showed that the sponge polypeptides must be grouped with the InsRs .
	manualset3
124741	1	405132	5	NULL	NULL	0	NULL	Phylogenetic analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analyses provided evidence for multiple spillover of DOBV-Aa to A. flavicollis , a crucial prerequisite for host switch and genetic reassortment .
	manualset3
124748	2	405132	5	NULL	NULL	0	NULL	evidence 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analyses provided evidence for multiple spillover of DOBV-Aa to A. flavicollis , a crucial prerequisite for host switch and genetic reassortment .
	manualset3
124759	3	405132	5	NULL	NULL	0	NULL	multiple spillover 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analyses provided evidence for multiple spillover of DOBV-Aa to A. flavicollis , a crucial prerequisite for host switch and genetic reassortment .
	manualset3
124768	4	405132	5	NULL	NULL	0	NULL	DOBV-Aa	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analyses provided evidence for multiple spillover of DOBV-Aa to A. flavicollis , a crucial prerequisite for host switch and genetic reassortment .
	manualset3
124770	5	405132	5	NULL	NULL	0	NULL	A. flavicollis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analyses provided evidence for multiple spillover of DOBV-Aa to A. flavicollis , a crucial prerequisite for host switch and genetic reassortment .
	manualset3
124784	6	405132	5	NULL	NULL	0	NULL	crucial prerequisite 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analyses provided evidence for multiple spillover of DOBV-Aa to A. flavicollis , a crucial prerequisite for host switch and genetic reassortment .
	manualset3
124786	7	405132	5	NULL	NULL	0	NULL	host switch	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analyses provided evidence for multiple spillover of DOBV-Aa to A. flavicollis , a crucial prerequisite for host switch and genetic reassortment .
	manualset3
124788	8	405132	5	NULL	NULL	0	NULL	genetic reassortment	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analyses provided evidence for multiple spillover of DOBV-Aa to A. flavicollis , a crucial prerequisite for host switch and genetic reassortment .
	manualset3
124791	1	405133	5	NULL	NULL	0	NULL	Phylogenetic analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis confirms the orthology of GFLO and FLO , and indicates that the gene may be useful for phylogenetic reconstruction at the genus or family level .
	manualset3
124793	2	405133	5	NULL	NULL	NULL	NULL	orthology 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis confirms the orthology of GFLO and FLO , and indicates that the gene may be useful for phylogenetic reconstruction at the genus or family level .
	manualset3
124805	3	405133	5	NULL	NULL	0	NULL	GFLO	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis confirms the orthology of GFLO and FLO , and indicates that the gene may be useful for phylogenetic reconstruction at the genus or family level .
	manualset3
124807	4	405133	5	NULL	NULL	0	NULL	FLO	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis confirms the orthology of GFLO and FLO , and indicates that the gene may be useful for phylogenetic reconstruction at the genus or family level .
	manualset3
124809	5	405133	5	NULL	NULL	0	NULL	gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis confirms the orthology of GFLO and FLO , and indicates that the gene may be useful for phylogenetic reconstruction at the genus or family level .
	manualset3
124817	6	405133	5	NULL	NULL	0	NULL	phylogenetic reconstruction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis confirms the orthology of GFLO and FLO , and indicates that the gene may be useful for phylogenetic reconstruction at the genus or family level .
	manualset3
124819	7	405133	5	NULL	NULL	0	NULL	genus or family level	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis confirms the orthology of GFLO and FLO , and indicates that the gene may be useful for phylogenetic reconstruction at the genus or family level .
	manualset3
124823	1	405134	5	NULL	NULL	0	NULL	Phylogenetic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis of 16S rRNA gene sequences showed that the two strains were closely related to one another ( 100 % similarity ) , and had the closest relationship with Microbacterium hominis NBRC 15708 ( T ) and Microbacterium insulae KCTC 19247 ( T ) ( 98.2-98 .3 % similarities ) .
	manualset3
124824	2	405134	5	NULL	NULL	0	NULL	16S rRNA gene sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis of 16S rRNA gene sequences showed that the two strains were closely related to one another ( 100 % similarity ) , and had the closest relationship with Microbacterium hominis NBRC 15708 ( T ) and Microbacterium insulae KCTC 19247 ( T ) ( 98.2-98 .3 % similarities ) .
	manualset3
124858	3	405134	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis of 16S rRNA gene sequences showed that the two strains were closely related to one another ( 100 % similarity ) , and had the closest relationship with Microbacterium hominis NBRC 15708 ( T ) and Microbacterium insulae KCTC 19247 ( T ) ( 98.2-98 .3 % similarities ) .
	manualset3
124859	4	405134	5	NULL	NULL	0	NULL	strains 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis of 16S rRNA gene sequences showed that the two strains were closely related to one another ( 100 % similarity ) , and had the closest relationship with Microbacterium hominis NBRC 15708 ( T ) and Microbacterium insulae KCTC 19247 ( T ) ( 98.2-98 .3 % similarities ) .
	manualset3
124860	5	405134	5	NULL	NULL	0	NULL	100 % similarity	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis of 16S rRNA gene sequences showed that the two strains were closely related to one another ( 100 % similarity ) , and had the closest relationship with Microbacterium hominis NBRC 15708 ( T ) and Microbacterium insulae KCTC 19247 ( T ) ( 98.2-98 .3 % similarities ) .
	manualset3
124861	6	405134	5	NULL	NULL	0	NULL	relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis of 16S rRNA gene sequences showed that the two strains were closely related to one another ( 100 % similarity ) , and had the closest relationship with Microbacterium hominis NBRC 15708 ( T ) and Microbacterium insulae KCTC 19247 ( T ) ( 98.2-98 .3 % similarities ) .
	manualset3
124862	7	405134	5	NULL	NULL	0	NULL	Microbacterium hominis NBRC 15708 ( T )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis of 16S rRNA gene sequences showed that the two strains were closely related to one another ( 100 % similarity ) , and had the closest relationship with Microbacterium hominis NBRC 15708 ( T ) and Microbacterium insulae KCTC 19247 ( T ) ( 98.2-98 .3 % similarities ) .
	manualset3
124863	8	405134	5	NULL	NULL	0	NULL	Microbacterium insulae KCTC 19247 ( T )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis of 16S rRNA gene sequences showed that the two strains were closely related to one another ( 100 % similarity ) , and had the closest relationship with Microbacterium hominis NBRC 15708 ( T ) and Microbacterium insulae KCTC 19247 ( T ) ( 98.2-98 .3 % similarities ) .
	manualset3
124864	9	405134	5	NULL	NULL	0	NULL	 98.2-98 .3 % similarities 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis of 16S rRNA gene sequences showed that the two strains were closely related to one another ( 100 % similarity ) , and had the closest relationship with Microbacterium hominis NBRC 15708 ( T ) and Microbacterium insulae KCTC 19247 ( T ) ( 98.2-98 .3 % similarities ) .
	manualset3
124865	1	405135	5	NULL	NULL	0	NULL	Phylogenetic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis of AtPPOX across all domains of life demonstrated that plant AtPPOX homologs have an additional Yjef_N domain preceding the Pyridox_Oxidase domain at the C-terminal end of the protein , while AtPPOX homologs from bacteria , fungi and animals have only Pyridox_Oxidase domain .
	manualset3
124866	2	405135	5	NULL	NULL	NULL	NULL	AtPPOX 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis of AtPPOX across all domains of life demonstrated that plant AtPPOX homologs have an additional Yjef_N domain preceding the Pyridox_Oxidase domain at the C-terminal end of the protein , while AtPPOX homologs from bacteria , fungi and animals have only Pyridox_Oxidase domain .
	manualset3
124867	3	405135	5	NULL	NULL	0	NULL	domains 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis of AtPPOX across all domains of life demonstrated that plant AtPPOX homologs have an additional Yjef_N domain preceding the Pyridox_Oxidase domain at the C-terminal end of the protein , while AtPPOX homologs from bacteria , fungi and animals have only Pyridox_Oxidase domain .
	manualset3
124868	4	405135	5	NULL	NULL	0	NULL	life 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis of AtPPOX across all domains of life demonstrated that plant AtPPOX homologs have an additional Yjef_N domain preceding the Pyridox_Oxidase domain at the C-terminal end of the protein , while AtPPOX homologs from bacteria , fungi and animals have only Pyridox_Oxidase domain .
	manualset3
124869	5	405135	5	NULL	NULL	NULL	NULL	plant AtPPOX homologs 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis of AtPPOX across all domains of life demonstrated that plant AtPPOX homologs have an additional Yjef_N domain preceding the Pyridox_Oxidase domain at the C-terminal end of the protein , while AtPPOX homologs from bacteria , fungi and animals have only Pyridox_Oxidase domain .
	manualset3
124870	6	405135	5	NULL	NULL	0	NULL	Yjef_N domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis of AtPPOX across all domains of life demonstrated that plant AtPPOX homologs have an additional Yjef_N domain preceding the Pyridox_Oxidase domain at the C-terminal end of the protein , while AtPPOX homologs from bacteria , fungi and animals have only Pyridox_Oxidase domain .
	manualset3
124871	7	405135	5	NULL	NULL	0	NULL	Pyridox_Oxidase domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis of AtPPOX across all domains of life demonstrated that plant AtPPOX homologs have an additional Yjef_N domain preceding the Pyridox_Oxidase domain at the C-terminal end of the protein , while AtPPOX homologs from bacteria , fungi and animals have only Pyridox_Oxidase domain .
	manualset3
124872	8	405135	5	NULL	NULL	0	NULL	C-terminal end	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis of AtPPOX across all domains of life demonstrated that plant AtPPOX homologs have an additional Yjef_N domain preceding the Pyridox_Oxidase domain at the C-terminal end of the protein , while AtPPOX homologs from bacteria , fungi and animals have only Pyridox_Oxidase domain .
	manualset3
124873	9	405135	5	NULL	NULL	0	NULL	protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis of AtPPOX across all domains of life demonstrated that plant AtPPOX homologs have an additional Yjef_N domain preceding the Pyridox_Oxidase domain at the C-terminal end of the protein , while AtPPOX homologs from bacteria , fungi and animals have only Pyridox_Oxidase domain .
	manualset3
124874	10	405135	5	NULL	NULL	0	NULL	AtPPOX homologs	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis of AtPPOX across all domains of life demonstrated that plant AtPPOX homologs have an additional Yjef_N domain preceding the Pyridox_Oxidase domain at the C-terminal end of the protein , while AtPPOX homologs from bacteria , fungi and animals have only Pyridox_Oxidase domain .
	manualset3
124875	11	405135	5	NULL	NULL	0	NULL	bacteria 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis of AtPPOX across all domains of life demonstrated that plant AtPPOX homologs have an additional Yjef_N domain preceding the Pyridox_Oxidase domain at the C-terminal end of the protein , while AtPPOX homologs from bacteria , fungi and animals have only Pyridox_Oxidase domain .
	manualset3
124876	12	405135	5	NULL	NULL	0	NULL	fungi 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis of AtPPOX across all domains of life demonstrated that plant AtPPOX homologs have an additional Yjef_N domain preceding the Pyridox_Oxidase domain at the C-terminal end of the protein , while AtPPOX homologs from bacteria , fungi and animals have only Pyridox_Oxidase domain .
	manualset3
124877	13	405135	5	NULL	NULL	0	NULL	animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis of AtPPOX across all domains of life demonstrated that plant AtPPOX homologs have an additional Yjef_N domain preceding the Pyridox_Oxidase domain at the C-terminal end of the protein , while AtPPOX homologs from bacteria , fungi and animals have only Pyridox_Oxidase domain .
	manualset3
124878	14	405135	5	NULL	NULL	0	NULL	Pyridox_Oxidase domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis of AtPPOX across all domains of life demonstrated that plant AtPPOX homologs have an additional Yjef_N domain preceding the Pyridox_Oxidase domain at the C-terminal end of the protein , while AtPPOX homologs from bacteria , fungi and animals have only Pyridox_Oxidase domain .
	manualset3
124879	1	405136	5	NULL	NULL	0	NULL	Phylogenetic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis of HLA alleles provided a basis for ethnic susceptibility to HTLV-1 infection and associated diseases , both ATL and HAM/TSP .
	manualset3
124880	2	405136	5	NULL	NULL	0	NULL	HLA alleles	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis of HLA alleles provided a basis for ethnic susceptibility to HTLV-1 infection and associated diseases , both ATL and HAM/TSP .
	manualset3
124881	3	405136	5	NULL	NULL	0	NULL	ethnic susceptibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis of HLA alleles provided a basis for ethnic susceptibility to HTLV-1 infection and associated diseases , both ATL and HAM/TSP .
	manualset3
124882	4	405136	5	NULL	NULL	0	NULL	HTLV-1 infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis of HLA alleles provided a basis for ethnic susceptibility to HTLV-1 infection and associated diseases , both ATL and HAM/TSP .
	manualset3
124883	5	405136	5	NULL	NULL	0	NULL	associated diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis of HLA alleles provided a basis for ethnic susceptibility to HTLV-1 infection and associated diseases , both ATL and HAM/TSP .
	manualset3
124884	6	405136	5	NULL	NULL	0	NULL	ATL 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis of HLA alleles provided a basis for ethnic susceptibility to HTLV-1 infection and associated diseases , both ATL and HAM/TSP .
	manualset3
124885	7	405136	5	NULL	NULL	0	NULL	HAM/TSP	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis of HLA alleles provided a basis for ethnic susceptibility to HTLV-1 infection and associated diseases , both ATL and HAM/TSP .
	manualset3
124886	1	405137	5	NULL	NULL	0	NULL	Phylogenetic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis revealed that these genes are distributed among seven orthology groups of the Hox gene family .
	manualset3
124887	2	405137	5	NULL	NULL	0	NULL	genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis revealed that these genes are distributed among seven orthology groups of the Hox gene family .
	manualset3
124888	3	405137	5	NULL	NULL	0	NULL	seven 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis revealed that these genes are distributed among seven orthology groups of the Hox gene family .
	manualset3
124889	4	405137	5	NULL	NULL	0	NULL	orthology groups	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis revealed that these genes are distributed among seven orthology groups of the Hox gene family .
	manualset3
124890	5	405137	5	NULL	NULL	0	NULL	Hox gene family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic analysis revealed that these genes are distributed among seven orthology groups of the Hox gene family .
	manualset3
124891	1	405138	5	NULL	NULL	0	NULL	Phylogenetic analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic and antigenic analyses demonstrated the diversity among H9 HA .
	manualset3
124892	2	405138	5	NULL	NULL	0	NULL	antigenic analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic and antigenic analyses demonstrated the diversity among H9 HA .
	manualset3
124893	3	405138	5	NULL	NULL	0	NULL	diversity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic and antigenic analyses demonstrated the diversity among H9 HA .
	manualset3
124894	4	405138	5	NULL	NULL	0	NULL	H9 HA	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogenetic and antigenic analyses demonstrated the diversity among H9 HA .
	manualset3
124895	1	405139	5	NULL	NULL	0	NULL	Phylogeny 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogeny of the defined murine microbiota : altered Schaedler flora .
	manualset3
124896	2	405139	5	NULL	NULL	0	NULL	murine microbiota	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogeny of the defined murine microbiota : altered Schaedler flora .
	manualset3
124897	3	405139	5	NULL	NULL	0	NULL	altered Schaedler flora	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogeny of the defined murine microbiota : altered Schaedler flora .
	manualset3
124898	1	405140	5	NULL	NULL	0	NULL	Phylogeographical analyses 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogeographical analyses based on the cpDNA network suggest that the present-day differentiation between western and eastern groups of H. pogonocalyx resulted from past fragmentation .
	manualset3
124899	2	405140	5	NULL	NULL	0	NULL	cpDNA network 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogeographical analyses based on the cpDNA network suggest that the present-day differentiation between western and eastern groups of H. pogonocalyx resulted from past fragmentation .
	manualset3
124900	3	405140	5	NULL	NULL	0	NULL	 present-day differentiation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogeographical analyses based on the cpDNA network suggest that the present-day differentiation between western and eastern groups of H. pogonocalyx resulted from past fragmentation .
	manualset3
124901	4	405140	5	NULL	NULL	0	NULL	 western and eastern groups of H. pogonocalyx	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogeographical analyses based on the cpDNA network suggest that the present-day differentiation between western and eastern groups of H. pogonocalyx resulted from past fragmentation .
	manualset3
124902	5	405140	5	NULL	NULL	0	NULL	past fragmentation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Phylogeographical analyses based on the cpDNA network suggest that the present-day differentiation between western and eastern groups of H. pogonocalyx resulted from past fragmentation .
	manualset3
124903	1	405141	5	NULL	NULL	0	NULL	Phyloproteomics 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Phyloproteomics employs two algorithms : a new parsing algorithm ( UNIPAL ) and a phylogenetic algorithm ( MIX ) .
	manualset3
124904	2	405141	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Phyloproteomics employs two algorithms : a new parsing algorithm ( UNIPAL ) and a phylogenetic algorithm ( MIX ) .
	manualset3
124905	3	405141	5	NULL	NULL	0	NULL	algorithms 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Phyloproteomics employs two algorithms : a new parsing algorithm ( UNIPAL ) and a phylogenetic algorithm ( MIX ) .
	manualset3
124906	4	405141	5	NULL	NULL	0	NULL	new parsing algorithm ( UNIPAL )	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Phyloproteomics employs two algorithms : a new parsing algorithm ( UNIPAL ) and a phylogenetic algorithm ( MIX ) .
	manualset3
124907	5	405141	5	NULL	NULL	0	NULL	phylogenetic algorithm ( MIX ) 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Phyloproteomics employs two algorithms : a new parsing algorithm ( UNIPAL ) and a phylogenetic algorithm ( MIX ) .
	manualset3
124908	1	405142	5	NULL	NULL	0	NULL	Physeal stapling	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Physeal stapling is the preferred method for GV correction , provided epiphyseal growth continues after stapling .
	manualset3
124909	2	405142	5	NULL	NULL	0	NULL	preferred method 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Physeal stapling is the preferred method for GV correction , provided epiphyseal growth continues after stapling .
	manualset3
124910	3	405142	5	NULL	NULL	0	NULL	GV correction 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Physeal stapling is the preferred method for GV correction , provided epiphyseal growth continues after stapling .
	manualset3
124911	4	405142	5	NULL	NULL	0	NULL	epiphyseal growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Physeal stapling is the preferred method for GV correction , provided epiphyseal growth continues after stapling .
	manualset3
124912	5	405142	5	NULL	NULL	0	NULL	stapling 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Physeal stapling is the preferred method for GV correction , provided epiphyseal growth continues after stapling .
	manualset3
124913	1	405143	5	NULL	NULL	0	NULL	Physical characterization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Physical and chemical characterization of Pt ( 12-n ) Cu ( n ) clusters via ab initio calculations .
	manualset3
124914	2	405143	5	NULL	NULL	0	NULL	chemical characterization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Physical and chemical characterization of Pt ( 12-n ) Cu ( n ) clusters via ab initio calculations .
	manualset3
124915	3	405143	5	NULL	NULL	0	NULL	Pt ( 12-n ) Cu ( n ) clusters	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Physical and chemical characterization of Pt ( 12-n ) Cu ( n ) clusters via ab initio calculations .
	manualset3
124916	4	405143	5	NULL	NULL	0	NULL	ab initio calculations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Physical and chemical characterization of Pt ( 12-n ) Cu ( n ) clusters via ab initio calculations .
	manualset3
124917	1	405144	5	NULL	NULL	0	NULL	Physical health	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Physical and emotional health of mothers of youth with functional abdominal pain .
	manualset3
124918	2	405144	5	NULL	NULL	0	NULL	emotional health	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Physical and emotional health of mothers of youth with functional abdominal pain .
	manualset3
124919	3	405144	5	NULL	NULL	0	NULL	mothers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Physical and emotional health of mothers of youth with functional abdominal pain .
	manualset3
124920	4	405144	5	NULL	NULL	0	NULL	youth 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Physical and emotional health of mothers of youth with functional abdominal pain .
	manualset3
124921	5	405144	5	NULL	NULL	0	NULL	functional abdominal pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Physical and emotional health of mothers of youth with functional abdominal pain .
	manualset3
124922	1	405145	5	NULL	NULL	0	NULL	Physical disruption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Physical disruption of the cell chains by ultrasonication produced similar single cells which were , however , noninvasive .
	manualset3
124923	2	405145	5	NULL	NULL	0	NULL	cell chains	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Physical disruption of the cell chains by ultrasonication produced similar single cells which were , however , noninvasive .
	manualset3
124924	3	405145	5	NULL	NULL	0	NULL	ultrasonication 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Physical disruption of the cell chains by ultrasonication produced similar single cells which were , however , noninvasive .
	manualset3
124925	4	405145	5	NULL	NULL	0	NULL	similar single cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Physical disruption of the cell chains by ultrasonication produced similar single cells which were , however , noninvasive .
	manualset3
124926	1	405146	5	NULL	NULL	0	NULL	Physical exercise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Physical exercise is associated with parasympathetic withdrawal and increased sympathetic activity resulting in heart rate increase .
	manualset3
124927	2	405146	5	NULL	NULL	0	NULL	parasympathetic withdrawal	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Physical exercise is associated with parasympathetic withdrawal and increased sympathetic activity resulting in heart rate increase .
	manualset3
124928	3	405146	5	NULL	NULL	0	NULL	increased sympathetic activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Physical exercise is associated with parasympathetic withdrawal and increased sympathetic activity resulting in heart rate increase .
	manualset3
124929	4	405146	5	NULL	NULL	0	NULL	heart rate increase	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Physical exercise is associated with parasympathetic withdrawal and increased sympathetic activity resulting in heart rate increase .
	manualset3
124930	1	405147	5	NULL	NULL	NULL	NULL	Physical interaction	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Physical interaction of full-length PS-1 and Go was also demonstrated .
	manualset3
124931	2	405147	5	NULL	NULL	0	NULL	full-length PS-1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Physical interaction of full-length PS-1 and Go was also demonstrated .
	manualset3
124932	3	405147	5	NULL	NULL	0	NULL	Go 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Physical interaction of full-length PS-1 and Go was also demonstrated .
	manualset3
124933	1	405148	5	NULL	NULL	0	NULL	high autopsy rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A high autopsy rate is required , even as regards sudden deaths that can not routinely be referred to as ischemic heart disease .
	manualset3
124934	2	405148	5	NULL	NULL	0	NULL	sudden deaths 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A high autopsy rate is required , even as regards sudden deaths that can not routinely be referred to as ischemic heart disease .
	manualset3
124935	3	405148	5	NULL	NULL	0	NULL	ischemic heart disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A high autopsy rate is required , even as regards sudden deaths that can not routinely be referred to as ischemic heart disease .
	manualset3
124936	1	405149	5	NULL	NULL	0	NULL	Physical working capacity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Physical working capacity and oxygen uptake at the anaerobic threshold ( 4 mmol/l blood lactate concentration ) increased from 68 + / - 12 to 80 + / - 16 watts and 0.95 + / - 0.14 to 1.10 + / - 0.20 l/min , respectively ( P & lt ; 0.01 ) .
	manualset3
124937	2	405149	5	NULL	NULL	0	NULL	oxygen uptake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Physical working capacity and oxygen uptake at the anaerobic threshold ( 4 mmol/l blood lactate concentration ) increased from 68 + / - 12 to 80 + / - 16 watts and 0.95 + / - 0.14 to 1.10 + / - 0.20 l/min , respectively ( P & lt ; 0.01 ) .
	manualset3
124938	3	405149	5	NULL	NULL	0	NULL	anaerobic threshold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Physical working capacity and oxygen uptake at the anaerobic threshold ( 4 mmol/l blood lactate concentration ) increased from 68 + / - 12 to 80 + / - 16 watts and 0.95 + / - 0.14 to 1.10 + / - 0.20 l/min , respectively ( P & lt ; 0.01 ) .
	manualset3
124939	4	405149	5	NULL	NULL	0	NULL	 4 mmol/l blood lactate concentration	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Physical working capacity and oxygen uptake at the anaerobic threshold ( 4 mmol/l blood lactate concentration ) increased from 68 + / - 12 to 80 + / - 16 watts and 0.95 + / - 0.14 to 1.10 + / - 0.20 l/min , respectively ( P & lt ; 0.01 ) .
	manualset3
124940	5	405149	5	NULL	NULL	0	NULL	68 + / - 12 to 80 + / - 16 watts	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Physical working capacity and oxygen uptake at the anaerobic threshold ( 4 mmol/l blood lactate concentration ) increased from 68 + / - 12 to 80 + / - 16 watts and 0.95 + / - 0.14 to 1.10 + / - 0.20 l/min , respectively ( P & lt ; 0.01 ) .
	manualset3
124941	6	405149	5	NULL	NULL	0	NULL	 0.95 + / - 0.14 to 1.10 + / - 0.20 l/min	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Physical working capacity and oxygen uptake at the anaerobic threshold ( 4 mmol/l blood lactate concentration ) increased from 68 + / - 12 to 80 + / - 16 watts and 0.95 + / - 0.14 to 1.10 + / - 0.20 l/min , respectively ( P & lt ; 0.01 ) .
	manualset3
124942	7	405149	5	NULL	NULL	0	NULL	 P & lt ; 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Physical working capacity and oxygen uptake at the anaerobic threshold ( 4 mmol/l blood lactate concentration ) increased from 68 + / - 12 to 80 + / - 16 watts and 0.95 + / - 0.14 to 1.10 + / - 0.20 l/min , respectively ( P & lt ; 0.01 ) .
	manualset3
124943	1	405150	5	NULL	NULL	0	NULL	Physicians 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Physicians and ATS service client hospitals value the Quality Indicator Process Reports .
	manualset3
124944	2	405150	5	NULL	NULL	0	NULL	ATS service client hospitals	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Physicians and ATS service client hospitals value the Quality Indicator Process Reports .
	manualset3
124945	3	405150	5	NULL	NULL	0	NULL	Quality Indicator Process Reports	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Physicians and ATS service client hospitals value the Quality Indicator Process Reports .
	manualset3
124946	1	405151	5	NULL	NULL	0	NULL	Physicians 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Physicians must be alert to the possibility of abuse within the family and home .
	manualset3
124948	3	405151	5	NULL	NULL	0	NULL	possibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Physicians must be alert to the possibility of abuse within the family and home .
	manualset3
124949	4	405151	5	NULL	NULL	0	NULL	abuse 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Physicians must be alert to the possibility of abuse within the family and home .
	manualset3
124950	5	405151	5	NULL	NULL	0	NULL	family 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Physicians must be alert to the possibility of abuse within the family and home .
	manualset3
124951	6	405151	5	NULL	NULL	0	NULL	home 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Physicians must be alert to the possibility of abuse within the family and home .
	manualset3
124952	1	405152	5	NULL	NULL	0	NULL	Physico-chemical characterization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Physico-chemical characterization further revealed that these precipitinogens can withstand ambient temperatures , but were sensitive to trypsin and ether whereas , chloroform had no effect on immunoprecipitation pattern of soluble antigens .
	manualset3
124953	2	405152	5	NULL	NULL	0	NULL	precipitinogens 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Physico-chemical characterization further revealed that these precipitinogens can withstand ambient temperatures , but were sensitive to trypsin and ether whereas , chloroform had no effect on immunoprecipitation pattern of soluble antigens .
	manualset3
124954	3	405152	5	NULL	NULL	0	NULL	ambient temperatures	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Physico-chemical characterization further revealed that these precipitinogens can withstand ambient temperatures , but were sensitive to trypsin and ether whereas , chloroform had no effect on immunoprecipitation pattern of soluble antigens .
	manualset3
124955	4	405152	5	NULL	NULL	0	NULL	trypsin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Physico-chemical characterization further revealed that these precipitinogens can withstand ambient temperatures , but were sensitive to trypsin and ether whereas , chloroform had no effect on immunoprecipitation pattern of soluble antigens .
	manualset3
124956	5	405152	5	NULL	NULL	0	NULL	ether 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Physico-chemical characterization further revealed that these precipitinogens can withstand ambient temperatures , but were sensitive to trypsin and ether whereas , chloroform had no effect on immunoprecipitation pattern of soluble antigens .
	manualset3
124957	6	405152	5	NULL	NULL	0	NULL	chloroform 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Physico-chemical characterization further revealed that these precipitinogens can withstand ambient temperatures , but were sensitive to trypsin and ether whereas , chloroform had no effect on immunoprecipitation pattern of soluble antigens .
	manualset3
124958	7	405152	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Physico-chemical characterization further revealed that these precipitinogens can withstand ambient temperatures , but were sensitive to trypsin and ether whereas , chloroform had no effect on immunoprecipitation pattern of soluble antigens .
	manualset3
124959	8	405152	5	NULL	NULL	0	NULL	immunoprecipitation pattern	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Physico-chemical characterization further revealed that these precipitinogens can withstand ambient temperatures , but were sensitive to trypsin and ether whereas , chloroform had no effect on immunoprecipitation pattern of soluble antigens .
	manualset3
124960	9	405152	5	NULL	NULL	0	NULL	soluble antigens	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Physico-chemical characterization further revealed that these precipitinogens can withstand ambient temperatures , but were sensitive to trypsin and ether whereas , chloroform had no effect on immunoprecipitation pattern of soluble antigens .
	manualset3
124961	1	405153	5	NULL	NULL	0	NULL	Physics 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Physics of thin-section MR imaging at low field strength .
	manualset3
124962	2	405153	5	NULL	NULL	0	NULL	thin-section MR imaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Physics of thin-section MR imaging at low field strength .
	manualset3
124963	3	405153	5	NULL	NULL	0	NULL	low field strength	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Physics of thin-section MR imaging at low field strength .
	manualset3
124964	1	405154	5	NULL	NULL	0	NULL	Physiologic alterations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiologic alterations induced by blood-warming during ether anesthesia .
	manualset3
124965	2	405154	5	NULL	NULL	0	NULL	blood-warming 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiologic alterations induced by blood-warming during ether anesthesia .
	manualset3
124966	3	405154	5	NULL	NULL	0	NULL	ether anesthesia	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiologic alterations induced by blood-warming during ether anesthesia .
	manualset3
124967	1	405155	5	NULL	NULL	0	NULL	Physiologic changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiologic changes that occur in patients with thyroid storm may lead to heparin resistance and inappropriate anticoagulation .
	manualset3
124968	2	405155	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiologic changes that occur in patients with thyroid storm may lead to heparin resistance and inappropriate anticoagulation .
	manualset3
124969	3	405155	5	NULL	NULL	0	NULL	thyroid storm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiologic changes that occur in patients with thyroid storm may lead to heparin resistance and inappropriate anticoagulation .
	manualset3
124970	4	405155	5	NULL	NULL	0	NULL	heparin resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiologic changes that occur in patients with thyroid storm may lead to heparin resistance and inappropriate anticoagulation .
	manualset3
124971	5	405155	5	NULL	NULL	0	NULL	inappropriate anticoagulation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiologic changes that occur in patients with thyroid storm may lead to heparin resistance and inappropriate anticoagulation .
	manualset3
124972	1	405156	5	NULL	NULL	0	NULL	high degree of convergence	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A high degree of convergence ( 82.6 % ) of somatic and visceral signals was revealed , as well as the interaction between the signals by the mutually blocking type .
	manualset3
124973	2	405156	5	NULL	NULL	0	NULL	82.6 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A high degree of convergence ( 82.6 % ) of somatic and visceral signals was revealed , as well as the interaction between the signals by the mutually blocking type .
	manualset3
124974	3	405156	5	NULL	NULL	0	NULL	somatic signals	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A high degree of convergence ( 82.6 % ) of somatic and visceral signals was revealed , as well as the interaction between the signals by the mutually blocking type .
	manualset3
124975	4	405156	5	NULL	NULL	0	NULL	visceral signals	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A high degree of convergence ( 82.6 % ) of somatic and visceral signals was revealed , as well as the interaction between the signals by the mutually blocking type .
	manualset3
124976	5	405156	5	NULL	NULL	0	NULL	interaction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A high degree of convergence ( 82.6 % ) of somatic and visceral signals was revealed , as well as the interaction between the signals by the mutually blocking type .
	manualset3
124977	6	405156	5	NULL	NULL	0	NULL	signals 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A high degree of convergence ( 82.6 % ) of somatic and visceral signals was revealed , as well as the interaction between the signals by the mutually blocking type .
	manualset3
124978	7	405156	5	NULL	NULL	0	NULL	mutually blocking type	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A high degree of convergence ( 82.6 % ) of somatic and visceral signals was revealed , as well as the interaction between the signals by the mutually blocking type .
	manualset3
124979	1	405157	5	NULL	NULL	0	NULL	Physiologic concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiologic concentrations of TGF-beta inhibited killing of intracellular L. chagasi in macrophages , although the phagocytosis-induced respiratory burst remained intact .
	manualset3
124980	2	405157	5	NULL	NULL	0	NULL	TGF-beta inhibited killing	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiologic concentrations of TGF-beta inhibited killing of intracellular L. chagasi in macrophages , although the phagocytosis-induced respiratory burst remained intact .
	manualset3
124981	3	405157	5	NULL	NULL	0	NULL	 intracellular L. chagasi 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiologic concentrations of TGF-beta inhibited killing of intracellular L. chagasi in macrophages , although the phagocytosis-induced respiratory burst remained intact .
	manualset3
124982	4	405157	5	NULL	NULL	0	NULL	macrophages 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiologic concentrations of TGF-beta inhibited killing of intracellular L. chagasi in macrophages , although the phagocytosis-induced respiratory burst remained intact .
	manualset3
125245	5	405157	5	NULL	NULL	0	NULL	phagocytosis-induced respiratory burst 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiologic concentrations of TGF-beta inhibited killing of intracellular L. chagasi in macrophages , although the phagocytosis-induced respiratory burst remained intact .
	manualset3
125246	1	405158	5	NULL	NULL	0	NULL	Physiological roles	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiological and pathological roles for microRNAs in the immune system .
	manualset3
125247	2	405158	5	NULL	NULL	0	NULL	pathological roles	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiological and pathological roles for microRNAs in the immune system .
	manualset3
125248	3	405158	5	NULL	NULL	0	NULL	microRNAs 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiological and pathological roles for microRNAs in the immune system .
	manualset3
125249	4	405158	5	NULL	NULL	0	NULL	immune system	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiological and pathological roles for microRNAs in the immune system .
	manualset3
125250	1	405159	5	NULL	NULL	0	NULL	Physiological effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiological effects of separation and reunion in relation to attachment and temperament in young children .
	manualset3
125251	2	405159	5	NULL	NULL	0	NULL	separation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiological effects of separation and reunion in relation to attachment and temperament in young children .
	manualset3
125252	3	405159	5	NULL	NULL	0	NULL	reunion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiological effects of separation and reunion in relation to attachment and temperament in young children .
	manualset3
125253	4	405159	5	NULL	NULL	0	NULL	relation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiological effects of separation and reunion in relation to attachment and temperament in young children .
	manualset3
125254	5	405159	5	NULL	NULL	0	NULL	attachment 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiological effects of separation and reunion in relation to attachment and temperament in young children .
	manualset3
125255	6	405159	5	NULL	NULL	0	NULL	temperament 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiological effects of separation and reunion in relation to attachment and temperament in young children .
	manualset3
125256	7	405159	5	NULL	NULL	0	NULL	young children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiological effects of separation and reunion in relation to attachment and temperament in young children .
	manualset3
125257	1	405160	5	NULL	NULL	0	NULL	Physiology 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiology of hypokinetic and hyperkinetic movement disorders : model for dyskinesia .
	manualset3
125258	2	405160	5	NULL	NULL	0	NULL	hypokinetic movement disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiology of hypokinetic and hyperkinetic movement disorders : model for dyskinesia .
	manualset3
125259	3	405160	5	NULL	NULL	0	NULL	hyperkinetic movement disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiology of hypokinetic and hyperkinetic movement disorders : model for dyskinesia .
	manualset3
125260	4	405160	5	NULL	NULL	0	NULL	model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiology of hypokinetic and hyperkinetic movement disorders : model for dyskinesia .
	manualset3
125261	5	405160	5	NULL	NULL	0	NULL	dyskinesia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiology of hypokinetic and hyperkinetic movement disorders : model for dyskinesia .
	manualset3
125310	1	405161	5	NULL	NULL	0	NULL	Physiotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiotherapy for 4 to 12 weeks produced improvement , but in four cases early operation for excision of fibrous tissue and lengthening of the triceps was necessary to restore adequate flexion .
	manualset3
125311	2	405161	5	NULL	NULL	0	NULL	4 to 12 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiotherapy for 4 to 12 weeks produced improvement , but in four cases early operation for excision of fibrous tissue and lengthening of the triceps was necessary to restore adequate flexion .
	manualset3
125312	3	405161	5	NULL	NULL	0	NULL	improvement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiotherapy for 4 to 12 weeks produced improvement , but in four cases early operation for excision of fibrous tissue and lengthening of the triceps was necessary to restore adequate flexion .
	manualset3
125320	4	405161	5	NULL	NULL	0	NULL	four	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiotherapy for 4 to 12 weeks produced improvement , but in four cases early operation for excision of fibrous tissue and lengthening of the triceps was necessary to restore adequate flexion .
	manualset3
125321	5	405161	5	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiotherapy for 4 to 12 weeks produced improvement , but in four cases early operation for excision of fibrous tissue and lengthening of the triceps was necessary to restore adequate flexion .
	manualset3
125324	6	405161	5	NULL	NULL	0	NULL	early operation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiotherapy for 4 to 12 weeks produced improvement , but in four cases early operation for excision of fibrous tissue and lengthening of the triceps was necessary to restore adequate flexion .
	manualset3
125327	7	405161	5	NULL	NULL	0	NULL	excision	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiotherapy for 4 to 12 weeks produced improvement , but in four cases early operation for excision of fibrous tissue and lengthening of the triceps was necessary to restore adequate flexion .
	manualset3
125328	8	405161	5	NULL	NULL	0	NULL	fibrous tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiotherapy for 4 to 12 weeks produced improvement , but in four cases early operation for excision of fibrous tissue and lengthening of the triceps was necessary to restore adequate flexion .
	manualset3
125331	9	405161	5	NULL	NULL	0	NULL	triceps	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiotherapy for 4 to 12 weeks produced improvement , but in four cases early operation for excision of fibrous tissue and lengthening of the triceps was necessary to restore adequate flexion .
	manualset3
125333	10	405161	5	NULL	NULL	0	NULL	flexion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiotherapy for 4 to 12 weeks produced improvement , but in four cases early operation for excision of fibrous tissue and lengthening of the triceps was necessary to restore adequate flexion .
	manualset3
125355	1	405162	5	NULL	NULL	0	NULL	Picornaviruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Picornaviruses , such as polio , translate their entire genome as a single polyprotein which must be proteolytically processed to produce the mature viral proteins .
	manualset3
125356	2	405162	5	NULL	NULL	NULL	NULL	polio	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Picornaviruses , such as polio , translate their entire genome as a single polyprotein which must be proteolytically processed to produce the mature viral proteins .
	manualset3
125357	3	405162	5	NULL	NULL	0	NULL	genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Picornaviruses , such as polio , translate their entire genome as a single polyprotein which must be proteolytically processed to produce the mature viral proteins .
	manualset3
125358	4	405162	5	NULL	NULL	0	NULL	single polyprotein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Picornaviruses , such as polio , translate their entire genome as a single polyprotein which must be proteolytically processed to produce the mature viral proteins .
	manualset3
125359	5	405162	5	NULL	NULL	0	NULL	mature viral proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Picornaviruses , such as polio , translate their entire genome as a single polyprotein which must be proteolytically processed to produce the mature viral proteins .
	manualset3
125360	1	405163	5	NULL	NULL	0	NULL	Piezoelectric-assisted removal	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Piezoelectric-assisted removal of a benign fibrous histiocytoma of the mandible : An innovative technique for prevention of dentoalveolar nerve injury .
	manualset3
125361	2	405163	5	NULL	NULL	0	NULL	benign fibrous histiocytoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Piezoelectric-assisted removal of a benign fibrous histiocytoma of the mandible : An innovative technique for prevention of dentoalveolar nerve injury .
	manualset3
125362	3	405163	5	NULL	NULL	0	NULL	mandible	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Piezoelectric-assisted removal of a benign fibrous histiocytoma of the mandible : An innovative technique for prevention of dentoalveolar nerve injury .
	manualset3
125363	4	405163	5	NULL	NULL	0	NULL	innovative technique	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Piezoelectric-assisted removal of a benign fibrous histiocytoma of the mandible : An innovative technique for prevention of dentoalveolar nerve injury .
	manualset3
125364	5	405163	5	NULL	NULL	0	NULL	prevention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Piezoelectric-assisted removal of a benign fibrous histiocytoma of the mandible : An innovative technique for prevention of dentoalveolar nerve injury .
	manualset3
125365	6	405163	5	NULL	NULL	0	NULL	dentoalveolar nerve injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Piezoelectric-assisted removal of a benign fibrous histiocytoma of the mandible : An innovative technique for prevention of dentoalveolar nerve injury .
	manualset3
125366	1	405164	5	NULL	NULL	0	NULL	Piezoelectric second generation lithotriptors	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Piezoelectric second generation lithotriptors are an established means of administering extracorporeal shockwave lithotripsy ( ESWL ) enabling treatment to be performed without anaesthesia or analgesia , but higher shockwave doses and multiple or staged treatment are frequently required .
	manualset3
125367	2	405164	5	NULL	NULL	0	NULL	 extracorporeal shockwave lithotripsy ( ESWL )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Piezoelectric second generation lithotriptors are an established means of administering extracorporeal shockwave lithotripsy ( ESWL ) enabling treatment to be performed without anaesthesia or analgesia , but higher shockwave doses and multiple or staged treatment are frequently required .
	manualset3
125368	3	405164	5	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Piezoelectric second generation lithotriptors are an established means of administering extracorporeal shockwave lithotripsy ( ESWL ) enabling treatment to be performed without anaesthesia or analgesia , but higher shockwave doses and multiple or staged treatment are frequently required .
	manualset3
125369	4	405164	5	NULL	NULL	0	NULL	anaesthesia	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Piezoelectric second generation lithotriptors are an established means of administering extracorporeal shockwave lithotripsy ( ESWL ) enabling treatment to be performed without anaesthesia or analgesia , but higher shockwave doses and multiple or staged treatment are frequently required .
	manualset3
125370	5	405164	5	NULL	NULL	0	NULL	analgesia	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Piezoelectric second generation lithotriptors are an established means of administering extracorporeal shockwave lithotripsy ( ESWL ) enabling treatment to be performed without anaesthesia or analgesia , but higher shockwave doses and multiple or staged treatment are frequently required .
	manualset3
125371	6	405164	5	NULL	NULL	0	NULL	higher shockwave doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Piezoelectric second generation lithotriptors are an established means of administering extracorporeal shockwave lithotripsy ( ESWL ) enabling treatment to be performed without anaesthesia or analgesia , but higher shockwave doses and multiple or staged treatment are frequently required .
	manualset3
125372	7	405164	5	NULL	NULL	0	NULL	multiple or staged treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Piezoelectric second generation lithotriptors are an established means of administering extracorporeal shockwave lithotripsy ( ESWL ) enabling treatment to be performed without anaesthesia or analgesia , but higher shockwave doses and multiple or staged treatment are frequently required .
	manualset3
125373	1	405165	5	NULL	NULL	0	NULL	Pigmented lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigmented lesion of the floor of oral cavity : what is your diagnosis ?
	manualset3
125374	2	405165	5	NULL	NULL	0	NULL	floor of oral cavity	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigmented lesion of the floor of oral cavity : what is your diagnosis ?
	manualset3
125375	3	405165	5	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigmented lesion of the floor of oral cavity : what is your diagnosis ?
	manualset3
125376	1	405166	5	NULL	NULL	0	NULL	Pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigs can also get infected or contaminated during transport , lairage or slaughter .
	manualset3
125377	2	405166	5	NULL	NULL	0	NULL	transport	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigs can also get infected or contaminated during transport , lairage or slaughter .
	manualset3
125378	3	405166	5	NULL	NULL	0	NULL	lairage	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigs can also get infected or contaminated during transport , lairage or slaughter .
	manualset3
125379	4	405166	5	NULL	NULL	0	NULL	slaughter	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigs can also get infected or contaminated during transport , lairage or slaughter .
	manualset3
125380	1	405167	5	NULL	NULL	0	NULL	Pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigs were fed a normal fat ( NF ) or high fat cholesterol ( HFC ) diet for 20-24 weeks .
	manualset3
125381	2	405167	5	NULL	NULL	0	NULL	normal fat ( NF ) diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigs were fed a normal fat ( NF ) or high fat cholesterol ( HFC ) diet for 20-24 weeks .
	manualset3
125382	3	405167	5	NULL	NULL	0	NULL	high fat cholesterol ( HFC ) diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigs were fed a normal fat ( NF ) or high fat cholesterol ( HFC ) diet for 20-24 weeks .
	manualset3
125383	4	405167	5	NULL	NULL	0	NULL	20-24 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigs were fed a normal fat ( NF ) or high fat cholesterol ( HFC ) diet for 20-24 weeks .
	manualset3
125384	1	405168	5	NULL	NULL	0	NULL	Pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigs were inoculated subcutaneously with live S. suis serotype 2 and blood was sampled before and on various days post inoculation ( p.i. ) , until the pigs were killed and autopsied on day 14 p.i. Clinical signs ( fever and lameness ) were observed in four of the five inoculated pigs from day 2 p.i. , and these pigs also had arthritic lesions at autopsy .
	manualset3
125385	2	405168	5	NULL	NULL	0	NULL	live S. suis serotype 2	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigs were inoculated subcutaneously with live S. suis serotype 2 and blood was sampled before and on various days post inoculation ( p.i. ) , until the pigs were killed and autopsied on day 14 p.i. Clinical signs ( fever and lameness ) were observed in four of the five inoculated pigs from day 2 p.i. , and these pigs also had arthritic lesions at autopsy .
	manualset3
125386	3	405168	5	NULL	NULL	0	NULL	blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigs were inoculated subcutaneously with live S. suis serotype 2 and blood was sampled before and on various days post inoculation ( p.i. ) , until the pigs were killed and autopsied on day 14 p.i. Clinical signs ( fever and lameness ) were observed in four of the five inoculated pigs from day 2 p.i. , and these pigs also had arthritic lesions at autopsy .
	manualset3
125387	4	405168	5	NULL	NULL	0	NULL	days	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigs were inoculated subcutaneously with live S. suis serotype 2 and blood was sampled before and on various days post inoculation ( p.i. ) , until the pigs were killed and autopsied on day 14 p.i. Clinical signs ( fever and lameness ) were observed in four of the five inoculated pigs from day 2 p.i. , and these pigs also had arthritic lesions at autopsy .
	manualset3
125388	5	405168	5	NULL	NULL	0	NULL	post inoculation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigs were inoculated subcutaneously with live S. suis serotype 2 and blood was sampled before and on various days post inoculation ( p.i. ) , until the pigs were killed and autopsied on day 14 p.i. Clinical signs ( fever and lameness ) were observed in four of the five inoculated pigs from day 2 p.i. , and these pigs also had arthritic lesions at autopsy .
	manualset3
125389	6	405168	5	NULL	NULL	0	NULL	pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigs were inoculated subcutaneously with live S. suis serotype 2 and blood was sampled before and on various days post inoculation ( p.i. ) , until the pigs were killed and autopsied on day 14 p.i. Clinical signs ( fever and lameness ) were observed in four of the five inoculated pigs from day 2 p.i. , and these pigs also had arthritic lesions at autopsy .
	manualset3
125390	7	405168	5	NULL	NULL	0	NULL	 day 14 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigs were inoculated subcutaneously with live S. suis serotype 2 and blood was sampled before and on various days post inoculation ( p.i. ) , until the pigs were killed and autopsied on day 14 p.i. Clinical signs ( fever and lameness ) were observed in four of the five inoculated pigs from day 2 p.i. , and these pigs also had arthritic lesions at autopsy .
	manualset3
125391	8	405168	5	NULL	NULL	0	NULL	Clinical signs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigs were inoculated subcutaneously with live S. suis serotype 2 and blood was sampled before and on various days post inoculation ( p.i. ) , until the pigs were killed and autopsied on day 14 p.i. Clinical signs ( fever and lameness ) were observed in four of the five inoculated pigs from day 2 p.i. , and these pigs also had arthritic lesions at autopsy .
	manualset3
125392	9	405168	5	NULL	NULL	0	NULL	fever	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigs were inoculated subcutaneously with live S. suis serotype 2 and blood was sampled before and on various days post inoculation ( p.i. ) , until the pigs were killed and autopsied on day 14 p.i. Clinical signs ( fever and lameness ) were observed in four of the five inoculated pigs from day 2 p.i. , and these pigs also had arthritic lesions at autopsy .
	manualset3
125393	10	405168	5	NULL	NULL	0	NULL	lameness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigs were inoculated subcutaneously with live S. suis serotype 2 and blood was sampled before and on various days post inoculation ( p.i. ) , until the pigs were killed and autopsied on day 14 p.i. Clinical signs ( fever and lameness ) were observed in four of the five inoculated pigs from day 2 p.i. , and these pigs also had arthritic lesions at autopsy .
	manualset3
125394	11	405168	5	NULL	NULL	0	NULL	four of the five 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigs were inoculated subcutaneously with live S. suis serotype 2 and blood was sampled before and on various days post inoculation ( p.i. ) , until the pigs were killed and autopsied on day 14 p.i. Clinical signs ( fever and lameness ) were observed in four of the five inoculated pigs from day 2 p.i. , and these pigs also had arthritic lesions at autopsy .
	manualset3
125395	12	405168	5	NULL	NULL	0	NULL	inoculated pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigs were inoculated subcutaneously with live S. suis serotype 2 and blood was sampled before and on various days post inoculation ( p.i. ) , until the pigs were killed and autopsied on day 14 p.i. Clinical signs ( fever and lameness ) were observed in four of the five inoculated pigs from day 2 p.i. , and these pigs also had arthritic lesions at autopsy .
	manualset3
125396	13	405168	5	NULL	NULL	0	NULL	day 2	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigs were inoculated subcutaneously with live S. suis serotype 2 and blood was sampled before and on various days post inoculation ( p.i. ) , until the pigs were killed and autopsied on day 14 p.i. Clinical signs ( fever and lameness ) were observed in four of the five inoculated pigs from day 2 p.i. , and these pigs also had arthritic lesions at autopsy .
	manualset3
125397	14	405168	5	NULL	NULL	0	NULL	pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigs were inoculated subcutaneously with live S. suis serotype 2 and blood was sampled before and on various days post inoculation ( p.i. ) , until the pigs were killed and autopsied on day 14 p.i. Clinical signs ( fever and lameness ) were observed in four of the five inoculated pigs from day 2 p.i. , and these pigs also had arthritic lesions at autopsy .
	manualset3
125398	15	405168	5	NULL	NULL	0	NULL	arthritic lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigs were inoculated subcutaneously with live S. suis serotype 2 and blood was sampled before and on various days post inoculation ( p.i. ) , until the pigs were killed and autopsied on day 14 p.i. Clinical signs ( fever and lameness ) were observed in four of the five inoculated pigs from day 2 p.i. , and these pigs also had arthritic lesions at autopsy .
	manualset3
125399	16	405168	5	NULL	NULL	0	NULL	autopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigs were inoculated subcutaneously with live S. suis serotype 2 and blood was sampled before and on various days post inoculation ( p.i. ) , until the pigs were killed and autopsied on day 14 p.i. Clinical signs ( fever and lameness ) were observed in four of the five inoculated pigs from day 2 p.i. , and these pigs also had arthritic lesions at autopsy .
	manualset3
125400	1	405169	5	NULL	NULL	0	NULL	Pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigs were provided with either .37 or .50 m2 per pig ( crowded ) and .60 or .74 m2 per pig ( uncrowded ) during the 55 to 91 and 91 to 127 kg weight periods , respectively .
	manualset3
125401	2	405169	5	NULL	NULL	0	NULL	.37 or .50 m2 per pig 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigs were provided with either .37 or .50 m2 per pig ( crowded ) and .60 or .74 m2 per pig ( uncrowded ) during the 55 to 91 and 91 to 127 kg weight periods , respectively .
	manualset3
125402	3	405169	5	NULL	NULL	0	NULL	.60 or .74 m2 per pig	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigs were provided with either .37 or .50 m2 per pig ( crowded ) and .60 or .74 m2 per pig ( uncrowded ) during the 55 to 91 and 91 to 127 kg weight periods , respectively .
	manualset3
125403	4	405169	5	NULL	NULL	0	NULL	55 to 91 and 91 to 127 kg weight periods	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pigs were provided with either .37 or .50 m2 per pig ( crowded ) and .60 or .74 m2 per pig ( uncrowded ) during the 55 to 91 and 91 to 127 kg weight periods , respectively .
	manualset3
125404	1	405170	5	NULL	NULL	0	NULL	Pilocytic astrocytoma ( PA )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pilocytic astrocytoma ( PA ) is the most frequently encountered glial tumor ( glioma or astrocytoma ) in children .
	manualset3
125405	2	405170	5	NULL	NULL	0	NULL	glial tumor ( glioma or astrocytoma )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pilocytic astrocytoma ( PA ) is the most frequently encountered glial tumor ( glioma or astrocytoma ) in children .
	manualset3
125406	3	405170	5	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Pilocytic astrocytoma ( PA ) is the most frequently encountered glial tumor ( glioma or astrocytoma ) in children .
	manualset3
125407	1	405171	5	NULL	NULL	0	NULL	Pin displacement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pin displacement was confirmed under fluoroscopic guidance and the clamp was used to withdraw the pin to the cutaneous entry point under CT ( step-by-step ) guidance .
	manualset3
125408	2	405171	5	NULL	NULL	NULL	NULL	fluoroscopic guidance	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pin displacement was confirmed under fluoroscopic guidance and the clamp was used to withdraw the pin to the cutaneous entry point under CT ( step-by-step ) guidance .
	manualset3
125409	3	405171	5	NULL	NULL	0	NULL	clamp	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Pin displacement was confirmed under fluoroscopic guidance and the clamp was used to withdraw the pin to the cutaneous entry point under CT ( step-by-step ) guidance .
	manualset3
125410	4	405171	5	NULL	NULL	0	NULL	pin	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Pin displacement was confirmed under fluoroscopic guidance and the clamp was used to withdraw the pin to the cutaneous entry point under CT ( step-by-step ) guidance .
	manualset3
125411	5	405171	5	NULL	NULL	0	NULL	cutaneous entry point	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pin displacement was confirmed under fluoroscopic guidance and the clamp was used to withdraw the pin to the cutaneous entry point under CT ( step-by-step ) guidance .
	manualset3
125412	6	405171	5	NULL	NULL	0	NULL	CT ( step-by-step ) guidance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pin displacement was confirmed under fluoroscopic guidance and the clamp was used to withdraw the pin to the cutaneous entry point under CT ( step-by-step ) guidance .
	manualset3
125413	1	405172	5	NULL	NULL	0	NULL	Pincher	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Pincher similarly mediates macroendocytosis for NGF ( TrkA ) and BDNF ( TrkB ) in both peripheral ( sympathetic ) and central ( hippocampal ) neurons .
	manualset3
125414	2	405172	5	NULL	NULL	0	NULL	macroendocytosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pincher similarly mediates macroendocytosis for NGF ( TrkA ) and BDNF ( TrkB ) in both peripheral ( sympathetic ) and central ( hippocampal ) neurons .
	manualset3
125415	3	405172	5	NULL	NULL	0	NULL	NGF ( TrkA )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Pincher similarly mediates macroendocytosis for NGF ( TrkA ) and BDNF ( TrkB ) in both peripheral ( sympathetic ) and central ( hippocampal ) neurons .
	manualset3
125416	4	405172	5	NULL	NULL	0	NULL	BDNF ( TrkB ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Pincher similarly mediates macroendocytosis for NGF ( TrkA ) and BDNF ( TrkB ) in both peripheral ( sympathetic ) and central ( hippocampal ) neurons .
	manualset3
125417	5	405172	5	NULL	NULL	0	NULL	peripheral ( sympathetic ) neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Pincher similarly mediates macroendocytosis for NGF ( TrkA ) and BDNF ( TrkB ) in both peripheral ( sympathetic ) and central ( hippocampal ) neurons .
	manualset3
125418	6	405172	5	NULL	NULL	0	NULL	central ( hippocampal ) neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Pincher similarly mediates macroendocytosis for NGF ( TrkA ) and BDNF ( TrkB ) in both peripheral ( sympathetic ) and central ( hippocampal ) neurons .
	manualset3
125419	1	405173	5	NULL	NULL	0	NULL	high density 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A high density of the leptin receptor was localized in the epithelia of the duct lumen .
	manualset3
125420	2	405173	5	NULL	NULL	0	NULL	leptin receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A high density of the leptin receptor was localized in the epithelia of the duct lumen .
	manualset3
125421	3	405173	5	NULL	NULL	0	NULL	epithelia	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	A high density of the leptin receptor was localized in the epithelia of the duct lumen .
	manualset3
125422	4	405173	5	NULL	NULL	0	NULL	duct lumen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A high density of the leptin receptor was localized in the epithelia of the duct lumen .
	manualset3
125423	1	405174	5	NULL	NULL	0	NULL	Pinealectomy results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pinealectomy results in a significant increase in lactate levels in rats subjected to an acute swimming exercise .
	manualset3
125424	2	405174	5	NULL	NULL	NULL	NULL	significant increase	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pinealectomy results in a significant increase in lactate levels in rats subjected to an acute swimming exercise .
	manualset3
125425	3	405174	5	NULL	NULL	0	NULL	lactate levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pinealectomy results in a significant increase in lactate levels in rats subjected to an acute swimming exercise .
	manualset3
125426	4	405174	5	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pinealectomy results in a significant increase in lactate levels in rats subjected to an acute swimming exercise .
	manualset3
125427	5	405174	5	NULL	NULL	0	NULL	acute swimming exercise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pinealectomy results in a significant increase in lactate levels in rats subjected to an acute swimming exercise .
	manualset3
125428	1	405175	5	NULL	NULL	0	NULL	Pink nodule	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pink nodule on the forearm : challenge .
	manualset3
125429	2	405175	5	NULL	NULL	0	NULL	forearm	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Pink nodule on the forearm : challenge .
	manualset3
125430	3	405175	5	NULL	NULL	0	NULL	challenge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pink nodule on the forearm : challenge .
	manualset3
125431	1	405176	5	NULL	NULL	0	NULL	Pioglitazone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pioglitazone inhibits the diabetogenic action of growth hormone , but not its ability to promote growth .
	manualset3
125432	2	405176	5	NULL	NULL	0	NULL	diabetogenic action	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pioglitazone inhibits the diabetogenic action of growth hormone , but not its ability to promote growth .
	manualset3
125433	3	405176	5	NULL	NULL	0	NULL	growth hormone	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Pioglitazone inhibits the diabetogenic action of growth hormone , but not its ability to promote growth .
	manualset3
125434	4	405176	5	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pioglitazone inhibits the diabetogenic action of growth hormone , but not its ability to promote growth .
	manualset3
125435	5	405176	5	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pioglitazone inhibits the diabetogenic action of growth hormone , but not its ability to promote growth .
	manualset3
125436	1	405177	5	NULL	NULL	0	NULL	Piroxicam	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Piroxicam is a nonsteroidal anti-inflammatory drug with low aqueous solubility which exhibits polymorphism .
	manualset3
125437	2	405177	5	NULL	NULL	0	NULL	nonsteroidal anti-inflammatory drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Piroxicam is a nonsteroidal anti-inflammatory drug with low aqueous solubility which exhibits polymorphism .
	manualset3
125438	3	405177	5	NULL	NULL	0	NULL	low aqueous solubility 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Piroxicam is a nonsteroidal anti-inflammatory drug with low aqueous solubility which exhibits polymorphism .
	manualset3
125439	4	405177	5	NULL	NULL	0	NULL	polymorphism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Piroxicam is a nonsteroidal anti-inflammatory drug with low aqueous solubility which exhibits polymorphism .
	manualset3
125440	1	405178	5	NULL	NULL	0	NULL	Pituitary GH absolute content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pituitary GH absolute content ( microgram/pituitary , not normalized with body weight ) increased slowly during gametogenesis and more abruptly in males during spermiation .
	manualset3
125441	2	405178	5	NULL	NULL	0	NULL	microgram/pituitary	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pituitary GH absolute content ( microgram/pituitary , not normalized with body weight ) increased slowly during gametogenesis and more abruptly in males during spermiation .
	manualset3
125442	3	405178	5	NULL	NULL	0	NULL	body weight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pituitary GH absolute content ( microgram/pituitary , not normalized with body weight ) increased slowly during gametogenesis and more abruptly in males during spermiation .
	manualset3
125443	4	405178	5	NULL	NULL	0	NULL	gametogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pituitary GH absolute content ( microgram/pituitary , not normalized with body weight ) increased slowly during gametogenesis and more abruptly in males during spermiation .
	manualset3
125444	5	405178	5	NULL	NULL	0	NULL	males	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pituitary GH absolute content ( microgram/pituitary , not normalized with body weight ) increased slowly during gametogenesis and more abruptly in males during spermiation .
	manualset3
125445	6	405178	5	NULL	NULL	0	NULL	spermiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pituitary GH absolute content ( microgram/pituitary , not normalized with body weight ) increased slowly during gametogenesis and more abruptly in males during spermiation .
	manualset3
125446	1	405179	5	NULL	NULL	0	NULL	Pituitary adenylate cyclase-activating polypeptide ( PACAP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Pituitary adenylate cyclase-activating polypeptide ( PACAP ) stimulates melatonin release from pineal cells and modulates glutamatergic regulation of the suprachiasmatic circadian clock in rodents .
	manualset3
125447	2	405179	5	NULL	NULL	0	NULL	melatonin release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pituitary adenylate cyclase-activating polypeptide ( PACAP ) stimulates melatonin release from pineal cells and modulates glutamatergic regulation of the suprachiasmatic circadian clock in rodents .
	manualset3
125448	3	405179	5	NULL	NULL	0	NULL	pineal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Pituitary adenylate cyclase-activating polypeptide ( PACAP ) stimulates melatonin release from pineal cells and modulates glutamatergic regulation of the suprachiasmatic circadian clock in rodents .
	manualset3
125449	4	405179	5	NULL	NULL	0	NULL	glutamatergic regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pituitary adenylate cyclase-activating polypeptide ( PACAP ) stimulates melatonin release from pineal cells and modulates glutamatergic regulation of the suprachiasmatic circadian clock in rodents .
	manualset3
125450	5	405179	5	NULL	NULL	0	NULL	suprachiasmatic circadian clock	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pituitary adenylate cyclase-activating polypeptide ( PACAP ) stimulates melatonin release from pineal cells and modulates glutamatergic regulation of the suprachiasmatic circadian clock in rodents .
	manualset3
125451	6	405179	5	NULL	NULL	0	NULL	rodents	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pituitary adenylate cyclase-activating polypeptide ( PACAP ) stimulates melatonin release from pineal cells and modulates glutamatergic regulation of the suprachiasmatic circadian clock in rodents .
	manualset3
125452	1	405180	5	NULL	NULL	0	NULL	high frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A high frequency of identify between some of the peptides suggests the possibility of gene duplication during the evolution of the structural gene for the enzyme .
	manualset3
125453	2	405180	5	NULL	NULL	0	NULL	peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	A high frequency of identify between some of the peptides suggests the possibility of gene duplication during the evolution of the structural gene for the enzyme .
	manualset3
125454	3	405180	5	NULL	NULL	0	NULL	possibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A high frequency of identify between some of the peptides suggests the possibility of gene duplication during the evolution of the structural gene for the enzyme .
	manualset3
125455	4	405180	5	NULL	NULL	0	NULL	gene duplication	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A high frequency of identify between some of the peptides suggests the possibility of gene duplication during the evolution of the structural gene for the enzyme .
	manualset3
125456	5	405180	5	NULL	NULL	0	NULL	evolution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A high frequency of identify between some of the peptides suggests the possibility of gene duplication during the evolution of the structural gene for the enzyme .
	manualset3
125457	6	405180	5	NULL	NULL	0	NULL	structural gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A high frequency of identify between some of the peptides suggests the possibility of gene duplication during the evolution of the structural gene for the enzyme .
	manualset3
125458	7	405180	5	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A high frequency of identify between some of the peptides suggests the possibility of gene duplication during the evolution of the structural gene for the enzyme .
	manualset3
125459	1	405181	5	NULL	NULL	0	NULL	Pituitary carcinoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pituitary carcinoma is a rare tumor characterized by poor responsiveness to therapy , leading to early death .
	manualset3
125460	2	405181	5	NULL	NULL	0	NULL	rare tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pituitary carcinoma is a rare tumor characterized by poor responsiveness to therapy , leading to early death .
	manualset3
125461	3	405181	5	NULL	NULL	0	NULL	poor responsiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pituitary carcinoma is a rare tumor characterized by poor responsiveness to therapy , leading to early death .
	manualset3
125462	4	405181	5	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pituitary carcinoma is a rare tumor characterized by poor responsiveness to therapy , leading to early death .
	manualset3
125463	5	405181	5	NULL	NULL	0	NULL	early death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pituitary carcinoma is a rare tumor characterized by poor responsiveness to therapy , leading to early death .
	manualset3
125464	1	405182	5	NULL	NULL	0	NULL	Plakophilin 1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Plakophilin 1 not only stimulated the recruitment of eIF4A1 into the cap complex but also its helicase activity .
	manualset3
125465	2	405182	5	NULL	NULL	0	NULL	recruitment	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Plakophilin 1 not only stimulated the recruitment of eIF4A1 into the cap complex but also its helicase activity .
	manualset3
125466	3	405182	5	NULL	NULL	0	NULL	eIF4A1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Plakophilin 1 not only stimulated the recruitment of eIF4A1 into the cap complex but also its helicase activity .
	manualset3
125467	4	405182	5	NULL	NULL	0	NULL	cap complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Plakophilin 1 not only stimulated the recruitment of eIF4A1 into the cap complex but also its helicase activity .
	manualset3
125468	5	405182	5	NULL	NULL	0	NULL	helicase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Plakophilin 1 not only stimulated the recruitment of eIF4A1 into the cap complex but also its helicase activity .
	manualset3
125469	1	405183	5	NULL	NULL	0	NULL	Planned and purposeful co-operation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Planned and purposeful co-operation between the surgeon and the physiotherapist is needed in the medical treatment of patients .
	manualset3
125470	2	405183	5	NULL	NULL	0	NULL	surgeon	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Planned and purposeful co-operation between the surgeon and the physiotherapist is needed in the medical treatment of patients .
	manualset3
125471	3	405183	5	NULL	NULL	0	NULL	physiotherapist	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Planned and purposeful co-operation between the surgeon and the physiotherapist is needed in the medical treatment of patients .
	manualset3
125472	4	405183	5	NULL	NULL	0	NULL	medical treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Planned and purposeful co-operation between the surgeon and the physiotherapist is needed in the medical treatment of patients .
	manualset3
125473	5	405183	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Planned and purposeful co-operation between the surgeon and the physiotherapist is needed in the medical treatment of patients .
	manualset3
125474	1	405184	5	NULL	NULL	0	NULL	Planning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Planning for recruitment advertising : Part 1 .
	manualset3
125475	2	405184	5	NULL	NULL	0	NULL	recruitment advertising	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Planning for recruitment advertising : Part 1 .
	manualset3
125476	3	405184	5	NULL	NULL	0	NULL	Part 1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Planning for recruitment advertising : Part 1 .
	manualset3
125477	1	405185	5	NULL	NULL	0	NULL	Planning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Planning the human resources for health is a complex process .
	manualset3
125478	2	405185	5	NULL	NULL	0	NULL	human resources	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Planning the human resources for health is a complex process .
	manualset3
125479	3	405185	5	NULL	NULL	0	NULL	health	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Planning the human resources for health is a complex process .
	manualset3
125480	4	405185	5	NULL	NULL	0	NULL	complex process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Planning the human resources for health is a complex process .
	manualset3
125481	1	405186	5	NULL	NULL	0	NULL	Plant-derived organic matter	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Plant-derived organic matter was not stored in soils , but was transformed to microbial remains , mainly in the form of carbohydrates and proteins and held in soil by organo-mineral interactions .
	manualset3
125483	2	405186	5	NULL	NULL	0	NULL	microbial remains	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Plant-derived organic matter was not stored in soils , but was transformed to microbial remains , mainly in the form of carbohydrates and proteins and held in soil by organo-mineral interactions .
	manualset3
125484	3	405186	5	NULL	NULL	0	NULL	carbohydrates	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Plant-derived organic matter was not stored in soils , but was transformed to microbial remains , mainly in the form of carbohydrates and proteins and held in soil by organo-mineral interactions .
	manualset3
125485	4	405186	5	NULL	NULL	0	NULL	proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Plant-derived organic matter was not stored in soils , but was transformed to microbial remains , mainly in the form of carbohydrates and proteins and held in soil by organo-mineral interactions .
	manualset3
125486	5	405186	5	NULL	NULL	0	NULL	soil	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Plant-derived organic matter was not stored in soils , but was transformed to microbial remains , mainly in the form of carbohydrates and proteins and held in soil by organo-mineral interactions .
	manualset3
125487	6	405186	5	NULL	NULL	0	NULL	organo-mineral interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Plant-derived organic matter was not stored in soils , but was transformed to microbial remains , mainly in the form of carbohydrates and proteins and held in soil by organo-mineral interactions .
	manualset3
125488	1	405187	5	NULL	NULL	0	NULL	Plant-growth-promoting rhizobacteria ( PGPR )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Plant-growth-promoting rhizobacteria ( PGPR ) are used on crops most often as seed treatments ; however , an alternative application method for transplanted vegetables is mixing PGPR into the soilless medium in which the transplants are grown .
	manualset3
125489	2	405187	5	NULL	NULL	0	NULL	crops	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Plant-growth-promoting rhizobacteria ( PGPR ) are used on crops most often as seed treatments ; however , an alternative application method for transplanted vegetables is mixing PGPR into the soilless medium in which the transplants are grown .
	manualset3
125490	3	405187	5	NULL	NULL	0	NULL	seed treatments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Plant-growth-promoting rhizobacteria ( PGPR ) are used on crops most often as seed treatments ; however , an alternative application method for transplanted vegetables is mixing PGPR into the soilless medium in which the transplants are grown .
	manualset3
125491	4	405187	5	NULL	NULL	0	NULL	alternative application method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Plant-growth-promoting rhizobacteria ( PGPR ) are used on crops most often as seed treatments ; however , an alternative application method for transplanted vegetables is mixing PGPR into the soilless medium in which the transplants are grown .
	manualset3
125492	5	405187	5	NULL	NULL	0	NULL	transplanted vegetables	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Plant-growth-promoting rhizobacteria ( PGPR ) are used on crops most often as seed treatments ; however , an alternative application method for transplanted vegetables is mixing PGPR into the soilless medium in which the transplants are grown .
	manualset3
125493	6	405187	5	NULL	NULL	0	NULL	PGPR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Plant-growth-promoting rhizobacteria ( PGPR ) are used on crops most often as seed treatments ; however , an alternative application method for transplanted vegetables is mixing PGPR into the soilless medium in which the transplants are grown .
	manualset3
125494	7	405187	5	NULL	NULL	0	NULL	soilless medium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Plant-growth-promoting rhizobacteria ( PGPR ) are used on crops most often as seed treatments ; however , an alternative application method for transplanted vegetables is mixing PGPR into the soilless medium in which the transplants are grown .
	manualset3
125495	8	405187	5	NULL	NULL	0	NULL	transplants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Plant-growth-promoting rhizobacteria ( PGPR ) are used on crops most often as seed treatments ; however , an alternative application method for transplanted vegetables is mixing PGPR into the soilless medium in which the transplants are grown .
	manualset3
125496	1	405188	5	NULL	NULL	0	NULL	Plant sterol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Plant sterol and stanols -- comparison and contrasts .
	manualset3
125497	2	405188	5	NULL	NULL	0	NULL	stanols	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Plant sterol and stanols -- comparison and contrasts .
	manualset3
125498	3	405188	5	NULL	NULL	0	NULL	comparison	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Plant sterol and stanols -- comparison and contrasts .
	manualset3
125499	4	405188	5	NULL	NULL	0	NULL	contrasts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Plant sterol and stanols -- comparison and contrasts .
	manualset3
125500	1	405189	5	NULL	NULL	0	NULL	high output process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A high output process can then be realized through high density culture .
	manualset3
125501	2	405189	5	NULL	NULL	0	NULL	high density culture	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A high output process can then be realized through high density culture .
	manualset3
125502	1	405190	5	NULL	NULL	0	NULL	Plantar ulcerations 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Plantar ulcerations of lichen planus are unusual manifestations that constrain the patient 's quality of life and are often refractory to treatment .
	manualset3
125503	2	405190	5	NULL	NULL	0	NULL	lichen planus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Plantar ulcerations of lichen planus are unusual manifestations that constrain the patient 's quality of life and are often refractory to treatment .
	manualset3
125504	3	405190	5	NULL	NULL	0	NULL	unusual manifestations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Plantar ulcerations of lichen planus are unusual manifestations that constrain the patient 's quality of life and are often refractory to treatment .
	manualset3
125505	4	405190	5	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Plantar ulcerations of lichen planus are unusual manifestations that constrain the patient 's quality of life and are often refractory to treatment .
	manualset3
125506	5	405190	5	NULL	NULL	0	NULL	quality of life	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Plantar ulcerations of lichen planus are unusual manifestations that constrain the patient 's quality of life and are often refractory to treatment .
	manualset3
125507	6	405190	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Plantar ulcerations of lichen planus are unusual manifestations that constrain the patient 's quality of life and are often refractory to treatment .
	manualset3
125508	1	405191	5	NULL	NULL	0	NULL	Plaques 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Plaques contained within arteries removed from three white males aged 51 , 55 and 70 are imaged in three-dimensions with monochromatic synchrotron x-ray radiation .
	manualset3
125509	2	405191	5	NULL	NULL	0	NULL	arteries 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Plaques contained within arteries removed from three white males aged 51 , 55 and 70 are imaged in three-dimensions with monochromatic synchrotron x-ray radiation .
	manualset3
125510	3	405191	5	NULL	NULL	0	NULL	 three	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Plaques contained within arteries removed from three white males aged 51 , 55 and 70 are imaged in three-dimensions with monochromatic synchrotron x-ray radiation .
	manualset3
125511	4	405191	5	NULL	NULL	0	NULL	white males	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Plaques contained within arteries removed from three white males aged 51 , 55 and 70 are imaged in three-dimensions with monochromatic synchrotron x-ray radiation .
	manualset3
125512	5	405191	5	NULL	NULL	0	NULL	51	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Plaques contained within arteries removed from three white males aged 51 , 55 and 70 are imaged in three-dimensions with monochromatic synchrotron x-ray radiation .
	manualset3
125513	6	405191	5	NULL	NULL	0	NULL	55	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Plaques contained within arteries removed from three white males aged 51 , 55 and 70 are imaged in three-dimensions with monochromatic synchrotron x-ray radiation .
	manualset3
125514	7	405191	5	NULL	NULL	0	NULL	70	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Plaques contained within arteries removed from three white males aged 51 , 55 and 70 are imaged in three-dimensions with monochromatic synchrotron x-ray radiation .
	manualset3
125515	8	405191	5	NULL	NULL	0	NULL	three-dimensions 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Plaques contained within arteries removed from three white males aged 51 , 55 and 70 are imaged in three-dimensions with monochromatic synchrotron x-ray radiation .
	manualset3
125516	9	405191	5	NULL	NULL	0	NULL	monochromatic synchrotron x-ray radiation	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Plaques contained within arteries removed from three white males aged 51 , 55 and 70 are imaged in three-dimensions with monochromatic synchrotron x-ray radiation .
	manualset3
125517	1	405192	5	NULL	NULL	0	NULL	Plasma AD	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma AD has been advocated for the screening and monitoring of cancer , as AD2 activity is increased in conditions associated with tumor growth .
	manualset3
125518	2	405192	5	NULL	NULL	0	NULL	screening 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma AD has been advocated for the screening and monitoring of cancer , as AD2 activity is increased in conditions associated with tumor growth .
	manualset3
125519	3	405192	5	NULL	NULL	0	NULL	monitoring 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma AD has been advocated for the screening and monitoring of cancer , as AD2 activity is increased in conditions associated with tumor growth .
	manualset3
125520	4	405192	5	NULL	NULL	0	NULL	cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma AD has been advocated for the screening and monitoring of cancer , as AD2 activity is increased in conditions associated with tumor growth .
	manualset3
125521	5	405192	5	NULL	NULL	NULL	NULL	AD2 activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Plasma AD has been advocated for the screening and monitoring of cancer , as AD2 activity is increased in conditions associated with tumor growth .
	manualset3
125522	6	405192	5	NULL	NULL	0	NULL	conditions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma AD has been advocated for the screening and monitoring of cancer , as AD2 activity is increased in conditions associated with tumor growth .
	manualset3
125523	7	405192	5	NULL	NULL	0	NULL	tumor growth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma AD has been advocated for the screening and monitoring of cancer , as AD2 activity is increased in conditions associated with tumor growth .
	manualset3
125524	1	405193	5	NULL	NULL	0	NULL	Plasma ADMA concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma ADMA concentrations increase markedly in hypertension .
	manualset3
125525	2	405193	5	NULL	NULL	0	NULL	hypertension 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma ADMA concentrations increase markedly in hypertension .
	manualset3
125526	1	405194	5	NULL	NULL	0	NULL	Plasma C-peptide concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma C-peptide concentrations increased from 0.11 + / - 0.02 to 1.73 + / - 0.04 nmol/l during C-peptide infusion .
	manualset3
125527	2	405194	5	NULL	NULL	0	NULL	0.11 + / - 0.02 nmol/l	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma C-peptide concentrations increased from 0.11 + / - 0.02 to 1.73 + / - 0.04 nmol/l during C-peptide infusion .
	manualset3
125528	3	405194	5	NULL	NULL	0	NULL	1.73 + / - 0.04 nmol/l 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma C-peptide concentrations increased from 0.11 + / - 0.02 to 1.73 + / - 0.04 nmol/l during C-peptide infusion .
	manualset3
125529	4	405194	5	NULL	NULL	0	NULL	C-peptide infusion	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma C-peptide concentrations increased from 0.11 + / - 0.02 to 1.73 + / - 0.04 nmol/l during C-peptide infusion .
	manualset3
125530	1	405195	5	NULL	NULL	0	NULL	Plasma HIV-1 RNA levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma HIV-1 RNA levels were inversely associated with A3G expression levels and with HI only among subjects who had HI & gt ; 1 .
	manualset3
125531	2	405195	5	NULL	NULL	0	NULL	A3G expression levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma HIV-1 RNA levels were inversely associated with A3G expression levels and with HI only among subjects who had HI & gt ; 1 .
	manualset3
125532	3	405195	5	NULL	NULL	0	NULL	HI	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma HIV-1 RNA levels were inversely associated with A3G expression levels and with HI only among subjects who had HI & gt ; 1 .
	manualset3
125533	4	405195	5	NULL	NULL	0	NULL	subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma HIV-1 RNA levels were inversely associated with A3G expression levels and with HI only among subjects who had HI & gt ; 1 .
	manualset3
125534	5	405195	5	NULL	NULL	0	NULL	 HI & gt ; 1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma HIV-1 RNA levels were inversely associated with A3G expression levels and with HI only among subjects who had HI & gt ; 1 .
	manualset3
125535	1	405196	5	NULL	NULL	0	NULL	CYTODIAGNOSIS 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( CYTODIAGNOSIS IN LUNG CANCER ) .
	manualset3
125536	2	405196	5	NULL	NULL	0	NULL	LUNG CANCER	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( CYTODIAGNOSIS IN LUNG CANCER ) .
	manualset3
125537	1	405197	5	NULL	NULL	0	NULL	Plasma TxB2	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma TxB2 rose minimally but significantly during maximal exercise , but 6-keto-PGF1 alpha did not change .
	manualset3
125538	2	405197	5	NULL	NULL	0	NULL	maximal exercise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma TxB2 rose minimally but significantly during maximal exercise , but 6-keto-PGF1 alpha did not change .
	manualset3
125539	3	405197	5	NULL	NULL	0	NULL	6-keto-PGF1 alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma TxB2 rose minimally but significantly during maximal exercise , but 6-keto-PGF1 alpha did not change .
	manualset3
125542	1	405198	5	NULL	NULL	0	NULL	Plasma cholesterol 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma and corpuscular cholesterol in sprue .
	manualset3
125543	2	405198	5	NULL	NULL	0	NULL	corpuscular cholesterol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma and corpuscular cholesterol in sprue .
	manualset3
125544	3	405198	5	NULL	NULL	0	NULL	sprue 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma and corpuscular cholesterol in sprue .
	manualset3
125545	1	405199	5	NULL	NULL	0	NULL	Plasma concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma concentrations of morphine , under the conditions of the present study , are not an objective indicator of pharmacological activity between one patient and another .
	manualset3
125546	2	405199	5	NULL	NULL	0	NULL	morphine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma concentrations of morphine , under the conditions of the present study , are not an objective indicator of pharmacological activity between one patient and another .
	manualset3
125547	3	405199	5	NULL	NULL	0	NULL	conditions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma concentrations of morphine , under the conditions of the present study , are not an objective indicator of pharmacological activity between one patient and another .
	manualset3
125548	4	405199	5	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma concentrations of morphine , under the conditions of the present study , are not an objective indicator of pharmacological activity between one patient and another .
	manualset3
125549	5	405199	5	NULL	NULL	0	NULL	objective indicator	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma concentrations of morphine , under the conditions of the present study , are not an objective indicator of pharmacological activity between one patient and another .
	manualset3
125550	6	405199	5	NULL	NULL	0	NULL	pharmacological activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma concentrations of morphine , under the conditions of the present study , are not an objective indicator of pharmacological activity between one patient and another .
	manualset3
125551	7	405199	5	NULL	NULL	0	NULL	one patient	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma concentrations of morphine , under the conditions of the present study , are not an objective indicator of pharmacological activity between one patient and another .
	manualset3
125552	1	405200	5	NULL	NULL	0	NULL	Plasma cortisol concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma cortisol concentrations were significantly higher with OC use at rest and during exercise at 45 and 65 % Vo ( 2 peak ) .
	manualset3
125553	2	405200	5	NULL	NULL	0	NULL	OC use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma cortisol concentrations were significantly higher with OC use at rest and during exercise at 45 and 65 % Vo ( 2 peak ) .
	manualset3
125554	3	405200	5	NULL	NULL	0	NULL	rest 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma cortisol concentrations were significantly higher with OC use at rest and during exercise at 45 and 65 % Vo ( 2 peak ) .
	manualset3
125555	4	405200	5	NULL	NULL	0	NULL	exercise 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma cortisol concentrations were significantly higher with OC use at rest and during exercise at 45 and 65 % Vo ( 2 peak ) .
	manualset3
125556	5	405200	5	NULL	NULL	0	NULL	45 and 65 % Vo ( 2 peak )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma cortisol concentrations were significantly higher with OC use at rest and during exercise at 45 and 65 % Vo ( 2 peak ) .
	manualset3
125570	1	405201	5	NULL	NULL	0	NULL	Plasma cortisol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma cortisol increased from 30 to 88 ng/ml 1 day after insertion of the cannula , to a maximum of 951 ng/ml 3 to 5 days after surgery , indicating the groupers were stressed by cannulation and post-cannulation inflammation .
	manualset3
125580	2	405201	5	NULL	NULL	0	NULL	30 to 88 ng/ml 1 day	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma cortisol increased from 30 to 88 ng/ml 1 day after insertion of the cannula , to a maximum of 951 ng/ml 3 to 5 days after surgery , indicating the groupers were stressed by cannulation and post-cannulation inflammation .
	manualset3
125588	3	405201	5	NULL	NULL	0	NULL	insertion 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma cortisol increased from 30 to 88 ng/ml 1 day after insertion of the cannula , to a maximum of 951 ng/ml 3 to 5 days after surgery , indicating the groupers were stressed by cannulation and post-cannulation inflammation .
	manualset3
125589	4	405201	5	NULL	NULL	0	NULL	cannula 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma cortisol increased from 30 to 88 ng/ml 1 day after insertion of the cannula , to a maximum of 951 ng/ml 3 to 5 days after surgery , indicating the groupers were stressed by cannulation and post-cannulation inflammation .
	manualset3
125590	5	405201	5	NULL	NULL	0	NULL	maximum 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma cortisol increased from 30 to 88 ng/ml 1 day after insertion of the cannula , to a maximum of 951 ng/ml 3 to 5 days after surgery , indicating the groupers were stressed by cannulation and post-cannulation inflammation .
	manualset3
125591	6	405201	5	NULL	NULL	0	NULL	951 ng/ml 3 to 5 days	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma cortisol increased from 30 to 88 ng/ml 1 day after insertion of the cannula , to a maximum of 951 ng/ml 3 to 5 days after surgery , indicating the groupers were stressed by cannulation and post-cannulation inflammation .
	manualset3
125592	7	405201	5	NULL	NULL	0	NULL	surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma cortisol increased from 30 to 88 ng/ml 1 day after insertion of the cannula , to a maximum of 951 ng/ml 3 to 5 days after surgery , indicating the groupers were stressed by cannulation and post-cannulation inflammation .
	manualset3
125593	8	405201	5	NULL	NULL	0	NULL	groupers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma cortisol increased from 30 to 88 ng/ml 1 day after insertion of the cannula , to a maximum of 951 ng/ml 3 to 5 days after surgery , indicating the groupers were stressed by cannulation and post-cannulation inflammation .
	manualset3
125594	9	405201	5	NULL	NULL	0	NULL	cannulation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma cortisol increased from 30 to 88 ng/ml 1 day after insertion of the cannula , to a maximum of 951 ng/ml 3 to 5 days after surgery , indicating the groupers were stressed by cannulation and post-cannulation inflammation .
	manualset3
125595	10	405201	5	NULL	NULL	0	NULL	post-cannulation inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma cortisol increased from 30 to 88 ng/ml 1 day after insertion of the cannula , to a maximum of 951 ng/ml 3 to 5 days after surgery , indicating the groupers were stressed by cannulation and post-cannulation inflammation .
	manualset3
125596	1	405202	5	NULL	NULL	0	NULL	 higher BMI-1 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A higher BMI-1 expression in CML CD34 ( + ) progenitors was associated with native BMI-1 immune responses .
	manualset3
125597	2	405202	5	NULL	NULL	0	NULL	CML CD34 ( + ) progenitors 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A higher BMI-1 expression in CML CD34 ( + ) progenitors was associated with native BMI-1 immune responses .
	manualset3
125598	3	405202	5	NULL	NULL	0	NULL	native BMI-1 immune responses	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A higher BMI-1 expression in CML CD34 ( + ) progenitors was associated with native BMI-1 immune responses .
	manualset3
125599	1	405203	5	NULL	NULL	0	NULL	Plasma growth hormone responses 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma growth hormone responses to growth hormone-releasing hormone in children of short stature .
	manualset3
125600	2	405203	5	NULL	NULL	0	NULL	growth hormone-releasing hormone	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma growth hormone responses to growth hormone-releasing hormone in children of short stature .
	manualset3
125601	3	405203	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma growth hormone responses to growth hormone-releasing hormone in children of short stature .
	manualset3
125602	4	405203	5	NULL	NULL	0	NULL	short stature	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma growth hormone responses to growth hormone-releasing hormone in children of short stature .
	manualset3
125607	1	405204	5	NULL	NULL	0	NULL	Plasma ionized Ca concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma ionized Ca concentrations prepartum and at calving in both cows and heifers increased with reduced DCAD in the diet .
	manualset3
125612	2	405204	5	NULL	NULL	0	NULL	prepartum 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma ionized Ca concentrations prepartum and at calving in both cows and heifers increased with reduced DCAD in the diet .
	manualset3
125615	3	405204	5	NULL	NULL	0	NULL	calving 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma ionized Ca concentrations prepartum and at calving in both cows and heifers increased with reduced DCAD in the diet .
	manualset3
125616	4	405204	5	NULL	NULL	0	NULL	cows 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma ionized Ca concentrations prepartum and at calving in both cows and heifers increased with reduced DCAD in the diet .
	manualset3
125617	5	405204	5	NULL	NULL	0	NULL	heifers 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma ionized Ca concentrations prepartum and at calving in both cows and heifers increased with reduced DCAD in the diet .
	manualset3
125618	6	405204	5	NULL	NULL	0	NULL	reduced DCAD	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma ionized Ca concentrations prepartum and at calving in both cows and heifers increased with reduced DCAD in the diet .
	manualset3
125619	7	405204	5	NULL	NULL	0	NULL	diet 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma ionized Ca concentrations prepartum and at calving in both cows and heifers increased with reduced DCAD in the diet .
	manualset3
125620	1	405205	5	NULL	NULL	0	NULL	Plasma lactate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma lactate increased 1.6 + / - 0.7 mM while riding 0.9 + / - 0.9 km.hr-1 faster .
	manualset3
125621	2	405205	5	NULL	NULL	0	NULL	1.6 + / - 0.7 mM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma lactate increased 1.6 + / - 0.7 mM while riding 0.9 + / - 0.9 km.hr-1 faster .
	manualset3
125622	3	405205	5	NULL	NULL	0	NULL	0.9 + / - 0.9 km.hr-1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma lactate increased 1.6 + / - 0.7 mM while riding 0.9 + / - 0.9 km.hr-1 faster .
	manualset3
125623	1	405206	5	NULL	NULL	0	NULL	Plasma leptin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma leptin in prepubertal patients with glycogen storage diseases .
	manualset3
125624	2	405206	5	NULL	NULL	0	NULL	prepubertal patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma leptin in prepubertal patients with glycogen storage diseases .
	manualset3
125625	3	405206	5	NULL	NULL	0	NULL	glycogen storage diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma leptin in prepubertal patients with glycogen storage diseases .
	manualset3
125626	1	405207	5	NULL	NULL	0	NULL	Plasma membrane Ca2 + ATPase isoform 4b	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma membrane Ca2 + ATPase isoform 4b binds to membrane-associated guanylate kinase ( MAGUK ) proteins via their PDZ ( PSD-95 / Dlg/ZO -1 ) domains .
	manualset3
125627	2	405207	5	NULL	NULL	0	NULL	membrane-associated guanylate kinase ( MAGUK ) proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma membrane Ca2 + ATPase isoform 4b binds to membrane-associated guanylate kinase ( MAGUK ) proteins via their PDZ ( PSD-95 / Dlg/ZO -1 ) domains .
	manualset3
125628	3	405207	5	NULL	NULL	0	NULL	PDZ ( PSD-95 / Dlg/ZO -1 ) domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma membrane Ca2 + ATPase isoform 4b binds to membrane-associated guanylate kinase ( MAGUK ) proteins via their PDZ ( PSD-95 / Dlg/ZO -1 ) domains .
	manualset3
125629	1	405208	5	NULL	NULL	0	NULL	Plasma or serum concentrations of SDF-1 protein	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma or serum concentrations of SDF-1 protein were measured by ELISA in samples from 31 HIV-1-seronegative individuals and 79 HIV-1-infected subjects .
	manualset3
125630	2	405208	5	NULL	NULL	0	NULL	ELISA 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma or serum concentrations of SDF-1 protein were measured by ELISA in samples from 31 HIV-1-seronegative individuals and 79 HIV-1-infected subjects .
	manualset3
125631	3	405208	5	NULL	NULL	NULL	NULL	samples 	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Plasma or serum concentrations of SDF-1 protein were measured by ELISA in samples from 31 HIV-1-seronegative individuals and 79 HIV-1-infected subjects .
	manualset3
125632	4	405208	5	NULL	NULL	0	NULL	31	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma or serum concentrations of SDF-1 protein were measured by ELISA in samples from 31 HIV-1-seronegative individuals and 79 HIV-1-infected subjects .
	manualset3
125633	5	405208	5	NULL	NULL	0	NULL	HIV-1-seronegative individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma or serum concentrations of SDF-1 protein were measured by ELISA in samples from 31 HIV-1-seronegative individuals and 79 HIV-1-infected subjects .
	manualset3
125634	6	405208	5	NULL	NULL	0	NULL	 79	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma or serum concentrations of SDF-1 protein were measured by ELISA in samples from 31 HIV-1-seronegative individuals and 79 HIV-1-infected subjects .
	manualset3
125635	7	405208	5	NULL	NULL	0	NULL	HIV-1-infected subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma or serum concentrations of SDF-1 protein were measured by ELISA in samples from 31 HIV-1-seronegative individuals and 79 HIV-1-infected subjects .
	manualset3
125636	1	405209	5	NULL	NULL	0	NULL	Plasma renin activity ( PRA ) 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma renin activity ( PRA ) was significantly elevated on the 1st day and remained at a high level until the 30th day .
	manualset3
125637	2	405209	5	NULL	NULL	0	NULL	1st day	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma renin activity ( PRA ) was significantly elevated on the 1st day and remained at a high level until the 30th day .
	manualset3
125638	3	405209	5	NULL	NULL	0	NULL	high level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma renin activity ( PRA ) was significantly elevated on the 1st day and remained at a high level until the 30th day .
	manualset3
125639	4	405209	5	NULL	NULL	0	NULL	30th day	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma renin activity ( PRA ) was significantly elevated on the 1st day and remained at a high level until the 30th day .
	manualset3
125640	1	405210	5	NULL	NULL	0	NULL	Plasma renin activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma renin activity fell during institution of bromocriptine and remained significantly lower during prolonged treatment .
	manualset3
125641	2	405210	5	NULL	NULL	0	NULL	institution 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma renin activity fell during institution of bromocriptine and remained significantly lower during prolonged treatment .
	manualset3
125642	3	405210	5	NULL	NULL	0	NULL	bromocriptine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma renin activity fell during institution of bromocriptine and remained significantly lower during prolonged treatment .
	manualset3
125643	4	405210	5	NULL	NULL	0	NULL	prolonged treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma renin activity fell during institution of bromocriptine and remained significantly lower during prolonged treatment .
	manualset3
125644	1	405211	5	NULL	NULL	0	NULL	higher proportion	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A higher proportion of men than women reported consuming runny eggs ( 12 % versus 8 % ) , pink hamburger ( 7 % versus 4 % ) , and raw oysters ( 2 % versus 0.4 % ) .
	manualset3
125645	2	405211	5	NULL	NULL	0	NULL	men 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A higher proportion of men than women reported consuming runny eggs ( 12 % versus 8 % ) , pink hamburger ( 7 % versus 4 % ) , and raw oysters ( 2 % versus 0.4 % ) .
	manualset3
125646	3	405211	5	NULL	NULL	0	NULL	women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A higher proportion of men than women reported consuming runny eggs ( 12 % versus 8 % ) , pink hamburger ( 7 % versus 4 % ) , and raw oysters ( 2 % versus 0.4 % ) .
	manualset3
125647	4	405211	5	NULL	NULL	0	NULL	runny eggs 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A higher proportion of men than women reported consuming runny eggs ( 12 % versus 8 % ) , pink hamburger ( 7 % versus 4 % ) , and raw oysters ( 2 % versus 0.4 % ) .
	manualset3
125648	5	405211	5	NULL	NULL	0	NULL	12 % versus 8 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A higher proportion of men than women reported consuming runny eggs ( 12 % versus 8 % ) , pink hamburger ( 7 % versus 4 % ) , and raw oysters ( 2 % versus 0.4 % ) .
	manualset3
125649	6	405211	5	NULL	NULL	0	NULL	pink hamburger	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A higher proportion of men than women reported consuming runny eggs ( 12 % versus 8 % ) , pink hamburger ( 7 % versus 4 % ) , and raw oysters ( 2 % versus 0.4 % ) .
	manualset3
125650	7	405211	5	NULL	NULL	0	NULL	7 % versus 4 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A higher proportion of men than women reported consuming runny eggs ( 12 % versus 8 % ) , pink hamburger ( 7 % versus 4 % ) , and raw oysters ( 2 % versus 0.4 % ) .
	manualset3
125651	8	405211	5	NULL	NULL	0	NULL	raw oysters 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A higher proportion of men than women reported consuming runny eggs ( 12 % versus 8 % ) , pink hamburger ( 7 % versus 4 % ) , and raw oysters ( 2 % versus 0.4 % ) .
	manualset3
125652	9	405211	5	NULL	NULL	0	NULL	2 % versus 0.4 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A higher proportion of men than women reported consuming runny eggs ( 12 % versus 8 % ) , pink hamburger ( 7 % versus 4 % ) , and raw oysters ( 2 % versus 0.4 % ) .
	manualset3
125653	1	405212	5	NULL	NULL	0	NULL	Plasma renin activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma renin activity was raised in all of 5 patients in whom it was measured , whereas aldosterone was raised in only 3 ; these results are similar to those found in ascites due to cirrhosis .
	manualset3
125654	2	405212	5	NULL	NULL	0	NULL	5	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma renin activity was raised in all of 5 patients in whom it was measured , whereas aldosterone was raised in only 3 ; these results are similar to those found in ascites due to cirrhosis .
	manualset3
125655	3	405212	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma renin activity was raised in all of 5 patients in whom it was measured , whereas aldosterone was raised in only 3 ; these results are similar to those found in ascites due to cirrhosis .
	manualset3
125656	4	405212	5	NULL	NULL	0	NULL	aldosterone 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma renin activity was raised in all of 5 patients in whom it was measured , whereas aldosterone was raised in only 3 ; these results are similar to those found in ascites due to cirrhosis .
	manualset3
125657	5	405212	5	NULL	NULL	0	NULL	3 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma renin activity was raised in all of 5 patients in whom it was measured , whereas aldosterone was raised in only 3 ; these results are similar to those found in ascites due to cirrhosis .
	manualset3
125658	6	405212	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma renin activity was raised in all of 5 patients in whom it was measured , whereas aldosterone was raised in only 3 ; these results are similar to those found in ascites due to cirrhosis .
	manualset3
125659	7	405212	5	NULL	NULL	0	NULL	ascites 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma renin activity was raised in all of 5 patients in whom it was measured , whereas aldosterone was raised in only 3 ; these results are similar to those found in ascites due to cirrhosis .
	manualset3
125660	8	405212	5	NULL	NULL	NULL	NULL	cirrhosis 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Plasma renin activity was raised in all of 5 patients in whom it was measured , whereas aldosterone was raised in only 3 ; these results are similar to those found in ascites due to cirrhosis .
	manualset3
125661	1	405213	5	NULL	NULL	0	NULL	Plasmatic concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasmatic concentration of glycemia and TNF - ( n = 10 ) were analyzed by the glucose oxidase and enzyme-linked immunosorbent assay method , respectively .
	manualset3
125662	2	405213	5	NULL	NULL	NULL	NULL	glycemia 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Plasmatic concentration of glycemia and TNF - ( n = 10 ) were analyzed by the glucose oxidase and enzyme-linked immunosorbent assay method , respectively .
	manualset3
125663	3	405213	5	NULL	NULL	0	NULL	TNF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasmatic concentration of glycemia and TNF - ( n = 10 ) were analyzed by the glucose oxidase and enzyme-linked immunosorbent assay method , respectively .
	manualset3
125664	4	405213	5	NULL	NULL	0	NULL	( n = 10 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasmatic concentration of glycemia and TNF - ( n = 10 ) were analyzed by the glucose oxidase and enzyme-linked immunosorbent assay method , respectively .
	manualset3
125665	5	405213	5	NULL	NULL	0	NULL	glucose oxidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasmatic concentration of glycemia and TNF - ( n = 10 ) were analyzed by the glucose oxidase and enzyme-linked immunosorbent assay method , respectively .
	manualset3
125666	6	405213	5	NULL	NULL	0	NULL	enzyme-linked immunosorbent assay method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasmatic concentration of glycemia and TNF - ( n = 10 ) were analyzed by the glucose oxidase and enzyme-linked immunosorbent assay method , respectively .
	manualset3
125667	1	405214	5	NULL	NULL	0	NULL	Plasmids pRAS3 .1	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasmids pRAS3 .1 and pRAS3 .2 are natural variants of the IncQ-2 plasmid family , that except for two differences , have identical plasmid backbones .
	manualset3
125668	2	405214	5	NULL	NULL	0	NULL	plasmid pRAS3 .2	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasmids pRAS3 .1 and pRAS3 .2 are natural variants of the IncQ-2 plasmid family , that except for two differences , have identical plasmid backbones .
	manualset3
125669	3	405214	5	NULL	NULL	0	NULL	natural variants	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasmids pRAS3 .1 and pRAS3 .2 are natural variants of the IncQ-2 plasmid family , that except for two differences , have identical plasmid backbones .
	manualset3
125670	4	405214	5	NULL	NULL	0	NULL	IncQ-2 plasmid family	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasmids pRAS3 .1 and pRAS3 .2 are natural variants of the IncQ-2 plasmid family , that except for two differences , have identical plasmid backbones .
	manualset3
125671	5	405214	5	NULL	NULL	0	NULL	two differences	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasmids pRAS3 .1 and pRAS3 .2 are natural variants of the IncQ-2 plasmid family , that except for two differences , have identical plasmid backbones .
	manualset3
125672	6	405214	5	NULL	NULL	0	NULL	identical plasmid backbones	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasmids pRAS3 .1 and pRAS3 .2 are natural variants of the IncQ-2 plasmid family , that except for two differences , have identical plasmid backbones .
	manualset3
125673	1	405215	5	NULL	NULL	0	NULL	Plasmin-coated B. burgdorferi 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasmin-coated B. burgdorferi degraded the purified ( ECM ) components fibronectin , laminin , and vitronectin , but not collagen .
	manualset3
125674	2	405215	5	NULL	NULL	0	NULL	 purified ( ECM ) components	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasmin-coated B. burgdorferi degraded the purified ( ECM ) components fibronectin , laminin , and vitronectin , but not collagen .
	manualset3
125675	3	405215	5	NULL	NULL	0	NULL	fibronectin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasmin-coated B. burgdorferi degraded the purified ( ECM ) components fibronectin , laminin , and vitronectin , but not collagen .
	manualset3
125676	4	405215	5	NULL	NULL	0	NULL	laminin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasmin-coated B. burgdorferi degraded the purified ( ECM ) components fibronectin , laminin , and vitronectin , but not collagen .
	manualset3
125677	5	405215	5	NULL	NULL	0	NULL	vitronectin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasmin-coated B. burgdorferi degraded the purified ( ECM ) components fibronectin , laminin , and vitronectin , but not collagen .
	manualset3
125678	6	405215	5	NULL	NULL	NULL	NULL	collagen 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Plasmin-coated B. burgdorferi degraded the purified ( ECM ) components fibronectin , laminin , and vitronectin , but not collagen .
	manualset3
125679	1	405216	5	NULL	NULL	0	NULL	Plasminogen 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasminogen and C-reactive protein increased significantly .
	manualset3
125680	2	405216	5	NULL	NULL	0	NULL	C-reactive protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasminogen and C-reactive protein increased significantly .
	manualset3
125681	1	405217	5	NULL	NULL	0	NULL	Plasminogen 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasminogen was identifiable in trophoblasts , and beta-2-microglobulin was uniformly absent from these cells .
	manualset3
125682	2	405217	5	NULL	NULL	0	NULL	trophoblasts 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasminogen was identifiable in trophoblasts , and beta-2-microglobulin was uniformly absent from these cells .
	manualset3
125683	3	405217	5	NULL	NULL	0	NULL	beta-2-microglobulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasminogen was identifiable in trophoblasts , and beta-2-microglobulin was uniformly absent from these cells .
	manualset3
125684	4	405217	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasminogen was identifiable in trophoblasts , and beta-2-microglobulin was uniformly absent from these cells .
	manualset3
125685	1	405218	5	NULL	NULL	0	NULL	Plastic surgery knowledge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Plastic surgery knowledge : state of the art .
	manualset3
125686	2	405218	5	NULL	NULL	0	NULL	state	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Plastic surgery knowledge : state of the art .
	manualset3
125687	3	405218	5	NULL	NULL	0	NULL	art 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Plastic surgery knowledge : state of the art .
	manualset3
125688	1	405219	5	NULL	NULL	0	NULL	highly conserved molecular switch	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A highly conserved molecular switch binds MSY-3 to regulate myogenin repression in postnatal muscle .
	manualset3
125689	2	405219	5	NULL	NULL	0	NULL	MSY-3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A highly conserved molecular switch binds MSY-3 to regulate myogenin repression in postnatal muscle .
	manualset3
125690	3	405219	5	NULL	NULL	0	NULL	myogenin repression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A highly conserved molecular switch binds MSY-3 to regulate myogenin repression in postnatal muscle .
	manualset3
125691	4	405219	5	NULL	NULL	0	NULL	postnatal muscle	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	A highly conserved molecular switch binds MSY-3 to regulate myogenin repression in postnatal muscle .
	manualset3
125692	1	405220	5	NULL	NULL	0	NULL	Plastics 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Plastics with enhanced fibronectin binding properties ( tissue culture plates ) were found to be hydrophilic and good substrates for cell attachment and growth while plastics with decreased fibronectin binding characteristics were found to be hydrophobic and poor substrates for cell attachment and growth .
	manualset3
125693	2	405220	5	NULL	NULL	0	NULL	fibronectin binding properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Plastics with enhanced fibronectin binding properties ( tissue culture plates ) were found to be hydrophilic and good substrates for cell attachment and growth while plastics with decreased fibronectin binding characteristics were found to be hydrophobic and poor substrates for cell attachment and growth .
	manualset3
125694	3	405220	5	NULL	NULL	0	NULL	tissue culture plates	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Plastics with enhanced fibronectin binding properties ( tissue culture plates ) were found to be hydrophilic and good substrates for cell attachment and growth while plastics with decreased fibronectin binding characteristics were found to be hydrophobic and poor substrates for cell attachment and growth .
	manualset3
125695	4	405220	5	NULL	NULL	0	NULL	good substrates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Plastics with enhanced fibronectin binding properties ( tissue culture plates ) were found to be hydrophilic and good substrates for cell attachment and growth while plastics with decreased fibronectin binding characteristics were found to be hydrophobic and poor substrates for cell attachment and growth .
	manualset3
125696	5	405220	5	NULL	NULL	0	NULL	cell attachment	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Plastics with enhanced fibronectin binding properties ( tissue culture plates ) were found to be hydrophilic and good substrates for cell attachment and growth while plastics with decreased fibronectin binding characteristics were found to be hydrophobic and poor substrates for cell attachment and growth .
	manualset3
125697	6	405220	5	NULL	NULL	0	NULL	growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Plastics with enhanced fibronectin binding properties ( tissue culture plates ) were found to be hydrophilic and good substrates for cell attachment and growth while plastics with decreased fibronectin binding characteristics were found to be hydrophobic and poor substrates for cell attachment and growth .
	manualset3
125698	7	405220	5	NULL	NULL	0	NULL	plastics 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Plastics with enhanced fibronectin binding properties ( tissue culture plates ) were found to be hydrophilic and good substrates for cell attachment and growth while plastics with decreased fibronectin binding characteristics were found to be hydrophobic and poor substrates for cell attachment and growth .
	manualset3
125699	8	405220	5	NULL	NULL	0	NULL	fibronectin binding characteristics 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Plastics with enhanced fibronectin binding properties ( tissue culture plates ) were found to be hydrophilic and good substrates for cell attachment and growth while plastics with decreased fibronectin binding characteristics were found to be hydrophobic and poor substrates for cell attachment and growth .
	manualset3
125700	9	405220	5	NULL	NULL	0	NULL	poor substrates 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Plastics with enhanced fibronectin binding properties ( tissue culture plates ) were found to be hydrophilic and good substrates for cell attachment and growth while plastics with decreased fibronectin binding characteristics were found to be hydrophobic and poor substrates for cell attachment and growth .
	manualset3
125701	10	405220	5	NULL	NULL	0	NULL	cell attachment 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Plastics with enhanced fibronectin binding properties ( tissue culture plates ) were found to be hydrophilic and good substrates for cell attachment and growth while plastics with decreased fibronectin binding characteristics were found to be hydrophobic and poor substrates for cell attachment and growth .
	manualset3
125702	11	405220	5	NULL	NULL	0	NULL	growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Plastics with enhanced fibronectin binding properties ( tissue culture plates ) were found to be hydrophilic and good substrates for cell attachment and growth while plastics with decreased fibronectin binding characteristics were found to be hydrophobic and poor substrates for cell attachment and growth .
	manualset3
125703	1	405221	5	NULL	NULL	0	NULL	Platelet-activating factor ( PAF )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet-activating factor ( PAF ) is a potent mediator of inflammation and is a mediator which is known to cause airway hyperresponsiveness in human and experimental animals .
	manualset3
125704	2	405221	5	NULL	NULL	0	NULL	potent mediator	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet-activating factor ( PAF ) is a potent mediator of inflammation and is a mediator which is known to cause airway hyperresponsiveness in human and experimental animals .
	manualset3
125705	3	405221	5	NULL	NULL	0	NULL	inflammation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet-activating factor ( PAF ) is a potent mediator of inflammation and is a mediator which is known to cause airway hyperresponsiveness in human and experimental animals .
	manualset3
125706	4	405221	5	NULL	NULL	0	NULL	mediator 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet-activating factor ( PAF ) is a potent mediator of inflammation and is a mediator which is known to cause airway hyperresponsiveness in human and experimental animals .
	manualset3
125707	5	405221	5	NULL	NULL	0	NULL	cause 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet-activating factor ( PAF ) is a potent mediator of inflammation and is a mediator which is known to cause airway hyperresponsiveness in human and experimental animals .
	manualset3
125708	6	405221	5	NULL	NULL	0	NULL	airway hyperresponsiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet-activating factor ( PAF ) is a potent mediator of inflammation and is a mediator which is known to cause airway hyperresponsiveness in human and experimental animals .
	manualset3
125709	7	405221	5	NULL	NULL	0	NULL	human 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet-activating factor ( PAF ) is a potent mediator of inflammation and is a mediator which is known to cause airway hyperresponsiveness in human and experimental animals .
	manualset3
125710	8	405221	5	NULL	NULL	0	NULL	experimental animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet-activating factor ( PAF ) is a potent mediator of inflammation and is a mediator which is known to cause airway hyperresponsiveness in human and experimental animals .
	manualset3
125711	1	405222	5	NULL	NULL	0	NULL	Platelet-activating factor 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet-activating factor has been implicated in a variety of disease processes including ischemic brain injury and endotoxic shock , but its effects on cerebral blood flow ( CBF ) and metabolism in normal brain have not been described .
	manualset3
125712	2	405222	5	NULL	NULL	0	NULL	disease processes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet-activating factor has been implicated in a variety of disease processes including ischemic brain injury and endotoxic shock , but its effects on cerebral blood flow ( CBF ) and metabolism in normal brain have not been described .
	manualset3
125713	3	405222	5	NULL	NULL	0	NULL	ischemic brain injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet-activating factor has been implicated in a variety of disease processes including ischemic brain injury and endotoxic shock , but its effects on cerebral blood flow ( CBF ) and metabolism in normal brain have not been described .
	manualset3
125714	4	405222	5	NULL	NULL	0	NULL	endotoxic shock	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet-activating factor has been implicated in a variety of disease processes including ischemic brain injury and endotoxic shock , but its effects on cerebral blood flow ( CBF ) and metabolism in normal brain have not been described .
	manualset3
125715	5	405222	5	NULL	NULL	0	NULL	effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet-activating factor has been implicated in a variety of disease processes including ischemic brain injury and endotoxic shock , but its effects on cerebral blood flow ( CBF ) and metabolism in normal brain have not been described .
	manualset3
125716	6	405222	5	NULL	NULL	0	NULL	cerebral blood flow ( CBF )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet-activating factor has been implicated in a variety of disease processes including ischemic brain injury and endotoxic shock , but its effects on cerebral blood flow ( CBF ) and metabolism in normal brain have not been described .
	manualset3
125717	7	405222	5	NULL	NULL	NULL	NULL	metabolism 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Platelet-activating factor has been implicated in a variety of disease processes including ischemic brain injury and endotoxic shock , but its effects on cerebral blood flow ( CBF ) and metabolism in normal brain have not been described .
	manualset3
125718	8	405222	5	NULL	NULL	0	NULL	normal brain 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet-activating factor has been implicated in a variety of disease processes including ischemic brain injury and endotoxic shock , but its effects on cerebral blood flow ( CBF ) and metabolism in normal brain have not been described .
	manualset3
125719	1	405223	5	NULL	NULL	0	NULL	Platelet-derived growth factor-BB 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet-derived growth factor-BB represses smooth muscle cell marker genes via changes in binding of MKL factors and histone deacetylases to their promoters .
	manualset3
125720	2	405223	5	NULL	NULL	0	NULL	smooth muscle cell marker genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet-derived growth factor-BB represses smooth muscle cell marker genes via changes in binding of MKL factors and histone deacetylases to their promoters .
	manualset3
125721	3	405223	5	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet-derived growth factor-BB represses smooth muscle cell marker genes via changes in binding of MKL factors and histone deacetylases to their promoters .
	manualset3
125722	4	405223	5	NULL	NULL	NULL	NULL	MKL factors	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Platelet-derived growth factor-BB represses smooth muscle cell marker genes via changes in binding of MKL factors and histone deacetylases to their promoters .
	manualset3
125723	5	405223	5	NULL	NULL	0	NULL	histone deacetylases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet-derived growth factor-BB represses smooth muscle cell marker genes via changes in binding of MKL factors and histone deacetylases to their promoters .
	manualset3
125724	6	405223	5	NULL	NULL	0	NULL	promoters 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet-derived growth factor-BB represses smooth muscle cell marker genes via changes in binding of MKL factors and histone deacetylases to their promoters .
	manualset3
125725	1	405224	5	NULL	NULL	0	NULL	Platelet adhesion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet adhesion to collagen : an update .
	manualset3
125726	2	405224	5	NULL	NULL	0	NULL	collagen 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet adhesion to collagen : an update .
	manualset3
125727	3	405224	5	NULL	NULL	0	NULL	update 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet adhesion to collagen : an update .
	manualset3
125728	1	405225	5	NULL	NULL	0	NULL	Platelet collagen interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet collagen interactions are initiated indirectly by interaction of platelet glycoprotein Ib ( GPIb ) with collagen-bound von Willebrand Factor ( vWF ) .
	manualset3
125729	2	405225	5	NULL	NULL	0	NULL	interaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet collagen interactions are initiated indirectly by interaction of platelet glycoprotein Ib ( GPIb ) with collagen-bound von Willebrand Factor ( vWF ) .
	manualset3
125730	3	405225	5	NULL	NULL	0	NULL	platelet glycoprotein Ib ( GPIb )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet collagen interactions are initiated indirectly by interaction of platelet glycoprotein Ib ( GPIb ) with collagen-bound von Willebrand Factor ( vWF ) .
	manualset3
125731	4	405225	5	NULL	NULL	0	NULL	collagen-bound von Willebrand Factor ( vWF )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet collagen interactions are initiated indirectly by interaction of platelet glycoprotein Ib ( GPIb ) with collagen-bound von Willebrand Factor ( vWF ) .
	manualset3
125732	1	405226	5	NULL	NULL	0	NULL	Platelet function profiles	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet function profiles in the elderly : results of a pharmacodynamic study in patients on clopidogrel therapy and effects of switching to prasugrel 5 mg in patients with high platelet reactivity .
	manualset3
125733	2	405226	5	NULL	NULL	0	NULL	elderly 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet function profiles in the elderly : results of a pharmacodynamic study in patients on clopidogrel therapy and effects of switching to prasugrel 5 mg in patients with high platelet reactivity .
	manualset3
125734	3	405226	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet function profiles in the elderly : results of a pharmacodynamic study in patients on clopidogrel therapy and effects of switching to prasugrel 5 mg in patients with high platelet reactivity .
	manualset3
125735	4	405226	5	NULL	NULL	0	NULL	pharmacodynamic study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet function profiles in the elderly : results of a pharmacodynamic study in patients on clopidogrel therapy and effects of switching to prasugrel 5 mg in patients with high platelet reactivity .
	manualset3
125736	5	405226	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet function profiles in the elderly : results of a pharmacodynamic study in patients on clopidogrel therapy and effects of switching to prasugrel 5 mg in patients with high platelet reactivity .
	manualset3
125737	6	405226	5	NULL	NULL	0	NULL	clopidogrel therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet function profiles in the elderly : results of a pharmacodynamic study in patients on clopidogrel therapy and effects of switching to prasugrel 5 mg in patients with high platelet reactivity .
	manualset3
125738	7	405226	5	NULL	NULL	0	NULL	effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet function profiles in the elderly : results of a pharmacodynamic study in patients on clopidogrel therapy and effects of switching to prasugrel 5 mg in patients with high platelet reactivity .
	manualset3
125739	8	405226	5	NULL	NULL	0	NULL	prasugrel 5 mg	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet function profiles in the elderly : results of a pharmacodynamic study in patients on clopidogrel therapy and effects of switching to prasugrel 5 mg in patients with high platelet reactivity .
	manualset3
125740	9	405226	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet function profiles in the elderly : results of a pharmacodynamic study in patients on clopidogrel therapy and effects of switching to prasugrel 5 mg in patients with high platelet reactivity .
	manualset3
125741	10	405226	5	NULL	NULL	0	NULL	high platelet reactivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet function profiles in the elderly : results of a pharmacodynamic study in patients on clopidogrel therapy and effects of switching to prasugrel 5 mg in patients with high platelet reactivity .
	manualset3
125742	1	405227	5	NULL	NULL	0	NULL	Platelet secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet secretion requires soluble N-ethylmaleimide-sensitive factor attachment protein ( SNAP ) receptor ( SNARE ) complex formation between different members of the syntaxin , SNAP-25 , and vesicle-associated membrane protein ( VAMP ) gene families .
	manualset3
125743	2	405227	5	NULL	NULL	0	NULL	 soluble N-ethylmaleimide-sensitive factor attachment protein ( SNAP ) receptor ( SNARE ) complex formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet secretion requires soluble N-ethylmaleimide-sensitive factor attachment protein ( SNAP ) receptor ( SNARE ) complex formation between different members of the syntaxin , SNAP-25 , and vesicle-associated membrane protein ( VAMP ) gene families .
	manualset3
125744	3	405227	5	NULL	NULL	0	NULL	members 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet secretion requires soluble N-ethylmaleimide-sensitive factor attachment protein ( SNAP ) receptor ( SNARE ) complex formation between different members of the syntaxin , SNAP-25 , and vesicle-associated membrane protein ( VAMP ) gene families .
	manualset3
125745	4	405227	5	NULL	NULL	0	NULL	syntaxin 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet secretion requires soluble N-ethylmaleimide-sensitive factor attachment protein ( SNAP ) receptor ( SNARE ) complex formation between different members of the syntaxin , SNAP-25 , and vesicle-associated membrane protein ( VAMP ) gene families .
	manualset3
125746	5	405227	5	NULL	NULL	0	NULL	SNAP-25	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet secretion requires soluble N-ethylmaleimide-sensitive factor attachment protein ( SNAP ) receptor ( SNARE ) complex formation between different members of the syntaxin , SNAP-25 , and vesicle-associated membrane protein ( VAMP ) gene families .
	manualset3
125747	6	405227	5	NULL	NULL	0	NULL	vesicle-associated membrane protein ( VAMP ) gene families	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet secretion requires soluble N-ethylmaleimide-sensitive factor attachment protein ( SNAP ) receptor ( SNARE ) complex formation between different members of the syntaxin , SNAP-25 , and vesicle-associated membrane protein ( VAMP ) gene families .
	manualset3
125748	1	405228	5	NULL	NULL	0	NULL	highly refined quality assurance program	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A highly refined quality assurance program relies on accurate outcome evaluations and the identification of patients who are truly worthy of peer review .
	manualset3
125749	2	405228	5	NULL	NULL	0	NULL	accurate outcome evaluations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A highly refined quality assurance program relies on accurate outcome evaluations and the identification of patients who are truly worthy of peer review .
	manualset3
125750	3	405228	5	NULL	NULL	0	NULL	identification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A highly refined quality assurance program relies on accurate outcome evaluations and the identification of patients who are truly worthy of peer review .
	manualset3
125751	4	405228	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A highly refined quality assurance program relies on accurate outcome evaluations and the identification of patients who are truly worthy of peer review .
	manualset3
125752	5	405228	5	NULL	NULL	0	NULL	peer review	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A highly refined quality assurance program relies on accurate outcome evaluations and the identification of patients who are truly worthy of peer review .
	manualset3
125753	1	405229	5	NULL	NULL	0	NULL	Platelet shape change	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet shape change ( percent discs and spheres ) was assayed by a light transmission technique .
	manualset3
125754	2	405229	5	NULL	NULL	0	NULL	 percent discs and spheres 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet shape change ( percent discs and spheres ) was assayed by a light transmission technique .
	manualset3
125755	3	405229	5	NULL	NULL	0	NULL	light transmission technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelet shape change ( percent discs and spheres ) was assayed by a light transmission technique .
	manualset3
125756	1	405230	5	NULL	NULL	0	NULL	Platelets 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelets contribute to blood coagulation at sites of vascular injury and to the recruitment of leukocytes at sites of inflammation .
	manualset3
125757	2	405230	5	NULL	NULL	0	NULL	 blood coagulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelets contribute to blood coagulation at sites of vascular injury and to the recruitment of leukocytes at sites of inflammation .
	manualset3
125758	3	405230	5	NULL	NULL	NULL	NULL	sites 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Platelets contribute to blood coagulation at sites of vascular injury and to the recruitment of leukocytes at sites of inflammation .
	manualset3
125759	4	405230	5	NULL	NULL	0	NULL	vascular injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelets contribute to blood coagulation at sites of vascular injury and to the recruitment of leukocytes at sites of inflammation .
	manualset3
125760	5	405230	5	NULL	NULL	0	NULL	recruitment 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelets contribute to blood coagulation at sites of vascular injury and to the recruitment of leukocytes at sites of inflammation .
	manualset3
125761	6	405230	5	NULL	NULL	0	NULL	leukocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelets contribute to blood coagulation at sites of vascular injury and to the recruitment of leukocytes at sites of inflammation .
	manualset3
125762	7	405230	5	NULL	NULL	0	NULL	sites 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelets contribute to blood coagulation at sites of vascular injury and to the recruitment of leukocytes at sites of inflammation .
	manualset3
125763	8	405230	5	NULL	NULL	0	NULL	inflammation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelets contribute to blood coagulation at sites of vascular injury and to the recruitment of leukocytes at sites of inflammation .
	manualset3
125764	1	405231	5	NULL	NULL	0	NULL	Platelets 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelets in plasma were activated by ADP and by collagen , and thrombin was used for the aggregation study of gel filtered platelets .
	manualset3
125765	2	405231	5	NULL	NULL	0	NULL	plasma 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelets in plasma were activated by ADP and by collagen , and thrombin was used for the aggregation study of gel filtered platelets .
	manualset3
125766	3	405231	5	NULL	NULL	0	NULL	ADP 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelets in plasma were activated by ADP and by collagen , and thrombin was used for the aggregation study of gel filtered platelets .
	manualset3
125767	4	405231	5	NULL	NULL	0	NULL	collagen 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelets in plasma were activated by ADP and by collagen , and thrombin was used for the aggregation study of gel filtered platelets .
	manualset3
125768	5	405231	5	NULL	NULL	0	NULL	thrombin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelets in plasma were activated by ADP and by collagen , and thrombin was used for the aggregation study of gel filtered platelets .
	manualset3
125769	6	405231	5	NULL	NULL	0	NULL	aggregation study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelets in plasma were activated by ADP and by collagen , and thrombin was used for the aggregation study of gel filtered platelets .
	manualset3
125770	7	405231	5	NULL	NULL	0	NULL	gel filtered platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Platelets in plasma were activated by ADP and by collagen , and thrombin was used for the aggregation study of gel filtered platelets .
	manualset3
125771	1	405232	5	NULL	NULL	0	NULL	Platypnea-orthodeoxia syndrome 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Platypnea-orthodeoxia syndrome : a rare complication after right pneumonectomy .
	manualset3
125772	2	405232	5	NULL	NULL	0	NULL	rare complication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Platypnea-orthodeoxia syndrome : a rare complication after right pneumonectomy .
	manualset3
125773	3	405232	5	NULL	NULL	0	NULL	right pneumonectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Platypnea-orthodeoxia syndrome : a rare complication after right pneumonectomy .
	manualset3
125774	1	405233	5	NULL	NULL	0	NULL	Play 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Play with parents is recognized as an important learning medium for all children , yet there have been remarkably few studies of mothers ' spontaneous actions with toys while playing with their children and none at all with Down 's syndrome infants .
	manualset3
125775	2	405233	5	NULL	NULL	0	NULL	parents 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Play with parents is recognized as an important learning medium for all children , yet there have been remarkably few studies of mothers ' spontaneous actions with toys while playing with their children and none at all with Down 's syndrome infants .
	manualset3
125776	3	405233	5	NULL	NULL	0	NULL	important learning medium	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Play with parents is recognized as an important learning medium for all children , yet there have been remarkably few studies of mothers ' spontaneous actions with toys while playing with their children and none at all with Down 's syndrome infants .
	manualset3
125777	4	405233	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Play with parents is recognized as an important learning medium for all children , yet there have been remarkably few studies of mothers ' spontaneous actions with toys while playing with their children and none at all with Down 's syndrome infants .
	manualset3
125778	5	405233	5	NULL	NULL	0	NULL	few studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Play with parents is recognized as an important learning medium for all children , yet there have been remarkably few studies of mothers ' spontaneous actions with toys while playing with their children and none at all with Down 's syndrome infants .
	manualset3
125779	6	405233	5	NULL	NULL	0	NULL	mothers ' spontaneous actions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Play with parents is recognized as an important learning medium for all children , yet there have been remarkably few studies of mothers ' spontaneous actions with toys while playing with their children and none at all with Down 's syndrome infants .
	manualset3
125780	7	405233	5	NULL	NULL	0	NULL	toys 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	Play with parents is recognized as an important learning medium for all children , yet there have been remarkably few studies of mothers ' spontaneous actions with toys while playing with their children and none at all with Down 's syndrome infants .
	manualset3
125781	8	405233	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Play with parents is recognized as an important learning medium for all children , yet there have been remarkably few studies of mothers ' spontaneous actions with toys while playing with their children and none at all with Down 's syndrome infants .
	manualset3
125782	9	405233	5	NULL	NULL	0	NULL	Down 's syndrome infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Play with parents is recognized as an important learning medium for all children , yet there have been remarkably few studies of mothers ' spontaneous actions with toys while playing with their children and none at all with Down 's syndrome infants .
	manualset3
125783	1	405234	5	NULL	NULL	0	NULL	Pleiotropic physiological consequences 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pleiotropic physiological consequences of feedback-insensitive phenylalanine biosynthesis in Arabidopsis thaliana .
	manualset3
125784	2	405234	5	NULL	NULL	0	NULL	feedback-insensitive phenylalanine biosynthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pleiotropic physiological consequences of feedback-insensitive phenylalanine biosynthesis in Arabidopsis thaliana .
	manualset3
125785	3	405234	5	NULL	NULL	0	NULL	Arabidopsis thaliana	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pleiotropic physiological consequences of feedback-insensitive phenylalanine biosynthesis in Arabidopsis thaliana .
	manualset3
125786	1	405235	5	NULL	NULL	0	NULL	Pleomorphic xanthoastrocytoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pleomorphic xanthoastrocytoma : report of 5 cases .
	manualset3
125787	2	405235	5	NULL	NULL	0	NULL	report 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Pleomorphic xanthoastrocytoma : report of 5 cases .
	manualset3
125788	3	405235	5	NULL	NULL	0	NULL	 5 cases	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pleomorphic xanthoastrocytoma : report of 5 cases .
	manualset3
125789	1	405236	5	NULL	NULL	0	NULL	Pleuropulmonary changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pleuropulmonary changes induced by ergoline drugs .
	manualset3
125790	2	405236	5	NULL	NULL	0	NULL	ergoline drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pleuropulmonary changes induced by ergoline drugs .
	manualset3
125791	1	405237	5	NULL	NULL	0	NULL	Plexins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Plexins are a family of single-pass transmembrane proteins that serve as cell surface receptors for Semaphorins during the embryonic development of animals .
	manualset3
125792	2	405237	5	NULL	NULL	0	NULL	family of single-pass transmembrane proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Plexins are a family of single-pass transmembrane proteins that serve as cell surface receptors for Semaphorins during the embryonic development of animals .
	manualset3
125793	3	405237	5	NULL	NULL	0	NULL	cell surface receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Plexins are a family of single-pass transmembrane proteins that serve as cell surface receptors for Semaphorins during the embryonic development of animals .
	manualset3
125794	4	405237	5	NULL	NULL	0	NULL	Semaphorins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Plexins are a family of single-pass transmembrane proteins that serve as cell surface receptors for Semaphorins during the embryonic development of animals .
	manualset3
125795	5	405237	5	NULL	NULL	0	NULL	embryonic development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Plexins are a family of single-pass transmembrane proteins that serve as cell surface receptors for Semaphorins during the embryonic development of animals .
	manualset3
125796	6	405237	5	NULL	NULL	0	NULL	animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Plexins are a family of single-pass transmembrane proteins that serve as cell surface receptors for Semaphorins during the embryonic development of animals .
	manualset3
125797	1	405238	5	NULL	NULL	0	NULL	highly sensitive and selective dopamine sensor	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A highly sensitive and selective dopamine sensor was fabricated with the unique 3D carbon nanotube nanoweb ( CNT-N ) electrode .
	manualset3
125798	2	405238	5	NULL	NULL	0	NULL	unique 3D carbon nanotube nanoweb ( CNT-N ) electrode	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A highly sensitive and selective dopamine sensor was fabricated with the unique 3D carbon nanotube nanoweb ( CNT-N ) electrode .
	manualset3
125799	1	405239	5	NULL	NULL	0	NULL	Plural light chains	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Plural light chains were simultaneously produced with the same heavy chain in a plasma cell by immunoelectron microscopy .
	manualset3
125800	2	405239	5	NULL	NULL	0	NULL	 heavy chain	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Plural light chains were simultaneously produced with the same heavy chain in a plasma cell by immunoelectron microscopy .
	manualset3
125801	3	405239	5	NULL	NULL	0	NULL	plasma cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Plural light chains were simultaneously produced with the same heavy chain in a plasma cell by immunoelectron microscopy .
	manualset3
125802	4	405239	5	NULL	NULL	0	NULL	immunoelectron microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Plural light chains were simultaneously produced with the same heavy chain in a plasma cell by immunoelectron microscopy .
	manualset3
125803	1	405240	5	NULL	NULL	0	NULL	Pluripotent embryonic stem ( ES ) cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Pluripotent embryonic stem ( ES ) cells can generate all cell types , but how cell lineages are initially specified and maintained during development remains largely unknown .
	manualset3
125804	2	405240	5	NULL	NULL	0	NULL	 cell types	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Pluripotent embryonic stem ( ES ) cells can generate all cell types , but how cell lineages are initially specified and maintained during development remains largely unknown .
	manualset3
125805	3	405240	5	NULL	NULL	0	NULL	cell lineages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Pluripotent embryonic stem ( ES ) cells can generate all cell types , but how cell lineages are initially specified and maintained during development remains largely unknown .
	manualset3
125806	4	405240	5	NULL	NULL	0	NULL	development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pluripotent embryonic stem ( ES ) cells can generate all cell types , but how cell lineages are initially specified and maintained during development remains largely unknown .
	manualset3
125807	1	405241	5	NULL	NULL	0	NULL	Pneumatization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pneumatization progresses gradually to reach at 16 years 23.0 + / -4.5 mm/22 .6 + / -5.8 mm/12 .8 + / -3.1 mm .
	manualset3
125808	2	405241	5	NULL	NULL	0	NULL	16 years 23.0 + / -4.5 mm/22 .6 + / -5.8 mm/12 .8 + / -3.1 mm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pneumatization progresses gradually to reach at 16 years 23.0 + / -4.5 mm/22 .6 + / -5.8 mm/12 .8 + / -3.1 mm .
	manualset3
125809	1	405242	5	NULL	NULL	0	NULL	Pneumatosis intestinalis ( PI )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pneumatosis intestinalis ( PI ) is an uncommon disorder defined as multiple foci of gas within the intestinal wall .
	manualset3
125810	2	405242	5	NULL	NULL	0	NULL	uncommon disorder	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pneumatosis intestinalis ( PI ) is an uncommon disorder defined as multiple foci of gas within the intestinal wall .
	manualset3
125811	3	405242	5	NULL	NULL	0	NULL	multiple foci of gas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pneumatosis intestinalis ( PI ) is an uncommon disorder defined as multiple foci of gas within the intestinal wall .
	manualset3
125812	4	405242	5	NULL	NULL	0	NULL	intestinal wall	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Pneumatosis intestinalis ( PI ) is an uncommon disorder defined as multiple foci of gas within the intestinal wall .
	manualset3
125813	1	405243	5	NULL	NULL	0	NULL	Pneumocystis prophylaxis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pneumocystis prophylaxis and survival in patients with advanced human immunodeficiency virus infection treated with zidovudine .
	manualset3
125814	2	405243	5	NULL	NULL	0	NULL	survival 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pneumocystis prophylaxis and survival in patients with advanced human immunodeficiency virus infection treated with zidovudine .
	manualset3
125815	3	405243	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Pneumocystis prophylaxis and survival in patients with advanced human immunodeficiency virus infection treated with zidovudine .
	manualset3
125816	4	405243	5	NULL	NULL	0	NULL	advanced human immunodeficiency virus infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pneumocystis prophylaxis and survival in patients with advanced human immunodeficiency virus infection treated with zidovudine .
	manualset3
125817	5	405243	5	NULL	NULL	0	NULL	zidovudine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pneumocystis prophylaxis and survival in patients with advanced human immunodeficiency virus infection treated with zidovudine .
	manualset3
125818	1	405244	5	NULL	NULL	0	NULL	Pneumoscrotum 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pneumoscrotum after jejunal perforation : a case report .
	manualset3
125819	2	405244	5	NULL	NULL	0	NULL	jejunal perforation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pneumoscrotum after jejunal perforation : a case report .
	manualset3
125820	3	405244	5	NULL	NULL	0	NULL	case report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Pneumoscrotum after jejunal perforation : a case report .
	manualset3
125821	1	405245	5	NULL	NULL	0	NULL	Pneumothorax detection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pneumothorax detection in emergency situations must be rapid and at the point of care .
	manualset3
125822	2	405245	5	NULL	NULL	0	NULL	emergency situations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pneumothorax detection in emergency situations must be rapid and at the point of care .
	manualset3
125823	3	405245	5	NULL	NULL	0	NULL	care 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pneumothorax detection in emergency situations must be rapid and at the point of care .
	manualset3
125824	1	405246	5	NULL	NULL	0	NULL	Podocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Podocytes respond to environmental cues by remodeling their slit diaphragms and cell-matrix adhesive junctions .
	manualset3
125825	2	405246	5	NULL	NULL	0	NULL	environmental cues	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Podocytes respond to environmental cues by remodeling their slit diaphragms and cell-matrix adhesive junctions .
	manualset3
125826	3	405246	5	NULL	NULL	0	NULL	remodeling 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Podocytes respond to environmental cues by remodeling their slit diaphragms and cell-matrix adhesive junctions .
	manualset3
125827	4	405246	5	NULL	NULL	0	NULL	slit diaphragms 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Podocytes respond to environmental cues by remodeling their slit diaphragms and cell-matrix adhesive junctions .
	manualset3
125828	5	405246	5	NULL	NULL	0	NULL	cell-matrix adhesive junctions 	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Podocytes respond to environmental cues by remodeling their slit diaphragms and cell-matrix adhesive junctions .
	manualset3
125829	1	405247	5	NULL	NULL	0	NULL	Point mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Point mutations in yeast CBF5 can abolish in vivo pseudouridylation of rRNA .
	manualset3
125830	2	405247	5	NULL	NULL	0	NULL	yeast CBF5 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Point mutations in yeast CBF5 can abolish in vivo pseudouridylation of rRNA .
	manualset3
125831	3	405247	5	NULL	NULL	0	NULL	pseudouridylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Point mutations in yeast CBF5 can abolish in vivo pseudouridylation of rRNA .
	manualset3
125832	4	405247	5	NULL	NULL	0	NULL	rRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Point mutations in yeast CBF5 can abolish in vivo pseudouridylation of rRNA .
	manualset3
125833	1	405248	5	NULL	NULL	0	NULL	highly sensitive derivatization method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A highly sensitive derivatization method for liquid chromatography ( LC ) - electrospray ionization ( ESI ) tandem mass spectrometry of dehydroepiandrosterone ( DHEA ) , testosterone ( T ) , pregnenolone ( P5 ) , and 17alpha-OH-pregnenolone ( 17-OHP5 ) was developed based on the use of fusaric acid as a reagent .
	manualset3
125834	2	405248	5	NULL	NULL	0	NULL	liquid chromatography (LC)-electrospray ionization (ESI) tandem mass spectrometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A highly sensitive derivatization method for liquid chromatography ( LC ) - electrospray ionization ( ESI ) tandem mass spectrometry of dehydroepiandrosterone ( DHEA ) , testosterone ( T ) , pregnenolone ( P5 ) , and 17alpha-OH-pregnenolone ( 17-OHP5 ) was developed based on the use of fusaric acid as a reagent .
	manualset3
125835	3	405248	5	NULL	NULL	0	NULL	dehydroepiandrosterone ( DHEA )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A highly sensitive derivatization method for liquid chromatography ( LC ) - electrospray ionization ( ESI ) tandem mass spectrometry of dehydroepiandrosterone ( DHEA ) , testosterone ( T ) , pregnenolone ( P5 ) , and 17alpha-OH-pregnenolone ( 17-OHP5 ) was developed based on the use of fusaric acid as a reagent .
	manualset3
125836	4	405248	5	NULL	NULL	0	NULL	testosterone ( T )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A highly sensitive derivatization method for liquid chromatography ( LC ) - electrospray ionization ( ESI ) tandem mass spectrometry of dehydroepiandrosterone ( DHEA ) , testosterone ( T ) , pregnenolone ( P5 ) , and 17alpha-OH-pregnenolone ( 17-OHP5 ) was developed based on the use of fusaric acid as a reagent .
	manualset3
125837	5	405248	5	NULL	NULL	NULL	NULL	pregnenolone ( P5 )	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A highly sensitive derivatization method for liquid chromatography ( LC ) - electrospray ionization ( ESI ) tandem mass spectrometry of dehydroepiandrosterone ( DHEA ) , testosterone ( T ) , pregnenolone ( P5 ) , and 17alpha-OH-pregnenolone ( 17-OHP5 ) was developed based on the use of fusaric acid as a reagent .
	manualset3
125838	6	405248	5	NULL	NULL	0	NULL	17alpha-OH-pregnenolone ( 17-OHP5 )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A highly sensitive derivatization method for liquid chromatography ( LC ) - electrospray ionization ( ESI ) tandem mass spectrometry of dehydroepiandrosterone ( DHEA ) , testosterone ( T ) , pregnenolone ( P5 ) , and 17alpha-OH-pregnenolone ( 17-OHP5 ) was developed based on the use of fusaric acid as a reagent .
	manualset3
125839	7	405248	5	NULL	NULL	0	NULL	fusaric acid 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A highly sensitive derivatization method for liquid chromatography ( LC ) - electrospray ionization ( ESI ) tandem mass spectrometry of dehydroepiandrosterone ( DHEA ) , testosterone ( T ) , pregnenolone ( P5 ) , and 17alpha-OH-pregnenolone ( 17-OHP5 ) was developed based on the use of fusaric acid as a reagent .
	manualset3
125840	8	405248	5	NULL	NULL	0	NULL	reagent 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A highly sensitive derivatization method for liquid chromatography ( LC ) - electrospray ionization ( ESI ) tandem mass spectrometry of dehydroepiandrosterone ( DHEA ) , testosterone ( T ) , pregnenolone ( P5 ) , and 17alpha-OH-pregnenolone ( 17-OHP5 ) was developed based on the use of fusaric acid as a reagent .
	manualset3
125841	1	405249	5	NULL	NULL	0	NULL	Polarity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Polarity was studied by approaches based on solvatochromic measurements and on the water effect on FTIR spectra .
	manualset3
125842	2	405249	5	NULL	NULL	0	NULL	approaches 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Polarity was studied by approaches based on solvatochromic measurements and on the water effect on FTIR spectra .
	manualset3
125843	3	405249	5	NULL	NULL	0	NULL	solvatochromic measurements 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Polarity was studied by approaches based on solvatochromic measurements and on the water effect on FTIR spectra .
	manualset3
125844	4	405249	5	NULL	NULL	0	NULL	water effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Polarity was studied by approaches based on solvatochromic measurements and on the water effect on FTIR spectra .
	manualset3
125845	5	405249	5	NULL	NULL	0	NULL	FTIR spectra	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Polarity was studied by approaches based on solvatochromic measurements and on the water effect on FTIR spectra .
	manualset3
125846	1	405250	5	NULL	NULL	0	NULL	Polarization 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Polarization of the one-cell C. elegans embryo establishes the animal 's anterior-posterior ( a-p ) axis .
	manualset3
125847	2	405250	5	NULL	NULL	0	NULL	one-cell C. elegans embryo	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Polarization of the one-cell C. elegans embryo establishes the animal 's anterior-posterior ( a-p ) axis .
	manualset3
125848	3	405250	5	NULL	NULL	0	NULL	animal 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Polarization of the one-cell C. elegans embryo establishes the animal 's anterior-posterior ( a-p ) axis .
	manualset3
125849	4	405250	5	NULL	NULL	0	NULL	anterior-posterior ( a-p ) axis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Polarization of the one-cell C. elegans embryo establishes the animal 's anterior-posterior ( a-p ) axis .
	manualset3
125850	1	405251	5	NULL	NULL	0	NULL	Pollen mother cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Pollen mother cells exposed to low dosages of x-rays at various stages show different frequencies of chromosome abnormalities in the first meiotic anaphase .
	manualset3
125851	2	405251	5	NULL	NULL	0	NULL	low dosages 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pollen mother cells exposed to low dosages of x-rays at various stages show different frequencies of chromosome abnormalities in the first meiotic anaphase .
	manualset3
125852	3	405251	5	NULL	NULL	0	NULL	 x-rays	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Pollen mother cells exposed to low dosages of x-rays at various stages show different frequencies of chromosome abnormalities in the first meiotic anaphase .
	manualset3
125853	4	405251	5	NULL	NULL	0	NULL	various stages 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Pollen mother cells exposed to low dosages of x-rays at various stages show different frequencies of chromosome abnormalities in the first meiotic anaphase .
	manualset3
125854	5	405251	5	NULL	NULL	0	NULL	frequencies 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pollen mother cells exposed to low dosages of x-rays at various stages show different frequencies of chromosome abnormalities in the first meiotic anaphase .
	manualset3
125855	6	405251	5	NULL	NULL	0	NULL	chromosome abnormalities 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pollen mother cells exposed to low dosages of x-rays at various stages show different frequencies of chromosome abnormalities in the first meiotic anaphase .
	manualset3
125856	7	405251	5	NULL	NULL	0	NULL	first meiotic anaphase	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Pollen mother cells exposed to low dosages of x-rays at various stages show different frequencies of chromosome abnormalities in the first meiotic anaphase .
	manualset3
125857	1	405252	5	NULL	NULL	0	NULL	Pollen 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Pollen of Cynodon dactylon ( Bermuda grass ) was present in nearly all the samples , and in a concurrent clinical study this antigen was found to be the most common cause of perennial rhinitis .
	manualset3
125858	2	405252	5	NULL	NULL	0	NULL	Cynodon dactylon ( Bermuda grass ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pollen of Cynodon dactylon ( Bermuda grass ) was present in nearly all the samples , and in a concurrent clinical study this antigen was found to be the most common cause of perennial rhinitis .
	manualset3
125859	3	405252	5	NULL	NULL	0	NULL	samples 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pollen of Cynodon dactylon ( Bermuda grass ) was present in nearly all the samples , and in a concurrent clinical study this antigen was found to be the most common cause of perennial rhinitis .
	manualset3
125860	4	405252	5	NULL	NULL	0	NULL	concurrent clinical study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pollen of Cynodon dactylon ( Bermuda grass ) was present in nearly all the samples , and in a concurrent clinical study this antigen was found to be the most common cause of perennial rhinitis .
	manualset3
125861	5	405252	5	NULL	NULL	0	NULL	antigen 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Pollen of Cynodon dactylon ( Bermuda grass ) was present in nearly all the samples , and in a concurrent clinical study this antigen was found to be the most common cause of perennial rhinitis .
	manualset3
125862	6	405252	5	NULL	NULL	0	NULL	cause 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pollen of Cynodon dactylon ( Bermuda grass ) was present in nearly all the samples , and in a concurrent clinical study this antigen was found to be the most common cause of perennial rhinitis .
	manualset3
125863	7	405252	5	NULL	NULL	0	NULL	perennial rhinitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pollen of Cynodon dactylon ( Bermuda grass ) was present in nearly all the samples , and in a concurrent clinical study this antigen was found to be the most common cause of perennial rhinitis .
	manualset3
125864	1	405253	5	NULL	NULL	0	NULL	Poly ( lactic-co-glycolic acid ) microsphere	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Poly ( lactic-co-glycolic acid ) microsphere as delivery system effectively maintains the blood concentration of huperzine A by a slow-release effect over a long time .
	manualset3
125865	2	405253	5	NULL	NULL	0	NULL	delivery system	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Poly ( lactic-co-glycolic acid ) microsphere as delivery system effectively maintains the blood concentration of huperzine A by a slow-release effect over a long time .
	manualset3
125866	3	405253	5	NULL	NULL	0	NULL	blood concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Poly ( lactic-co-glycolic acid ) microsphere as delivery system effectively maintains the blood concentration of huperzine A by a slow-release effect over a long time .
	manualset3
125867	4	405253	5	NULL	NULL	0	NULL	huperzine A	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Poly ( lactic-co-glycolic acid ) microsphere as delivery system effectively maintains the blood concentration of huperzine A by a slow-release effect over a long time .
	manualset3
125868	5	405253	5	NULL	NULL	0	NULL	slow-release effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Poly ( lactic-co-glycolic acid ) microsphere as delivery system effectively maintains the blood concentration of huperzine A by a slow-release effect over a long time .
	manualset3
125869	6	405253	5	NULL	NULL	0	NULL	long time	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Poly ( lactic-co-glycolic acid ) microsphere as delivery system effectively maintains the blood concentration of huperzine A by a slow-release effect over a long time .
	manualset3
125870	1	405254	5	NULL	NULL	0	NULL	Poly ( ( 3-hydroxyoctanoate ) - co - ( 3-hydroxyundecenoate ) ) ( PHOU ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Poly ( ( 3-hydroxyoctanoate ) - co - ( 3-hydroxyundecenoate ) ) ( PHOU ) was first methanolyzed and its unsaturated side chains were quantitatively oxidized to carboxylic acid .
	manualset3
125871	2	405254	5	NULL	NULL	0	NULL	unsaturated side chains 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Poly ( ( 3-hydroxyoctanoate ) - co - ( 3-hydroxyundecenoate ) ) ( PHOU ) was first methanolyzed and its unsaturated side chains were quantitatively oxidized to carboxylic acid .
	manualset3
125872	3	405254	5	NULL	NULL	0	NULL	carboxylic acid 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Poly ( ( 3-hydroxyoctanoate ) - co - ( 3-hydroxyundecenoate ) ) ( PHOU ) was first methanolyzed and its unsaturated side chains were quantitatively oxidized to carboxylic acid .
	manualset3
125873	1	405255	5	NULL	NULL	0	NULL	Poly ( A ) ( 40 ) tails	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Poly ( A ) ( 40 ) tails were added to the 3 ' end of the genome to stabilize the transcribed RNA .
	manualset3
125874	2	405255	5	NULL	NULL	0	NULL	3 ' end 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Poly ( A ) ( 40 ) tails were added to the 3 ' end of the genome to stabilize the transcribed RNA .
	manualset3
125875	3	405255	5	NULL	NULL	0	NULL	genome 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Poly ( A ) ( 40 ) tails were added to the 3 ' end of the genome to stabilize the transcribed RNA .
	manualset3
125876	4	405255	5	NULL	NULL	0	NULL	transcribed RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Poly ( A ) ( 40 ) tails were added to the 3 ' end of the genome to stabilize the transcribed RNA .
	manualset3
125877	1	405256	5	NULL	NULL	0	NULL	Poly ( N-isopropyl acrylamide ) or pNIPAM	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Poly ( N-isopropyl acrylamide ) or pNIPAM is a thermoresponsive polymer that is widely studied for use in bioengineering applications .
	manualset3
125878	2	405256	5	NULL	NULL	0	NULL	thermoresponsive polymer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Poly ( N-isopropyl acrylamide ) or pNIPAM is a thermoresponsive polymer that is widely studied for use in bioengineering applications .
	manualset3
125879	3	405256	5	NULL	NULL	0	NULL	use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Poly ( N-isopropyl acrylamide ) or pNIPAM is a thermoresponsive polymer that is widely studied for use in bioengineering applications .
	manualset3
125880	4	405256	5	NULL	NULL	0	NULL	bioengineering applications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Poly ( N-isopropyl acrylamide ) or pNIPAM is a thermoresponsive polymer that is widely studied for use in bioengineering applications .
	manualset3
125881	1	405257	5	NULL	NULL	0	NULL	Poly ( lactide-co-glycolide ) nanoparticles	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Poly ( lactide-co-glycolide ) nanoparticles loaded with pilocarpine hydrochloride were prepared by the high-pressure emulsification-solvent evaporation method .
	manualset3
125882	2	405257	5	NULL	NULL	0	NULL	pilocarpine hydrochloride	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Poly ( lactide-co-glycolide ) nanoparticles loaded with pilocarpine hydrochloride were prepared by the high-pressure emulsification-solvent evaporation method .
	manualset3
125883	3	405257	5	NULL	NULL	0	NULL	high-pressure emulsification-solvent evaporation method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Poly ( lactide-co-glycolide ) nanoparticles loaded with pilocarpine hydrochloride were prepared by the high-pressure emulsification-solvent evaporation method .
	manualset3
125884	1	405258	5	NULL	NULL	0	NULL	Polyacrylamide ( PAA ) - bentonite ( B ) and zeolite ( Z ) composites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyacrylamide ( PAA ) - bentonite ( B ) and zeolite ( Z ) composites were prepared by direct polymerization of PAA in suspensions of B and Z. Phytate ( Phy ) immobilized onto the composites to obtain their Phy modifications .
	manualset3
125885	2	405258	5	NULL	NULL	0	NULL	direct polymerization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyacrylamide ( PAA ) - bentonite ( B ) and zeolite ( Z ) composites were prepared by direct polymerization of PAA in suspensions of B and Z. Phytate ( Phy ) immobilized onto the composites to obtain their Phy modifications .
	manualset3
125886	3	405258	5	NULL	NULL	0	NULL	PAA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyacrylamide ( PAA ) - bentonite ( B ) and zeolite ( Z ) composites were prepared by direct polymerization of PAA in suspensions of B and Z. Phytate ( Phy ) immobilized onto the composites to obtain their Phy modifications .
	manualset3
125887	4	405258	5	NULL	NULL	0	NULL	suspensions 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyacrylamide ( PAA ) - bentonite ( B ) and zeolite ( Z ) composites were prepared by direct polymerization of PAA in suspensions of B and Z. Phytate ( Phy ) immobilized onto the composites to obtain their Phy modifications .
	manualset3
125888	5	405258	5	NULL	NULL	0	NULL	B 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyacrylamide ( PAA ) - bentonite ( B ) and zeolite ( Z ) composites were prepared by direct polymerization of PAA in suspensions of B and Z. Phytate ( Phy ) immobilized onto the composites to obtain their Phy modifications .
	manualset3
125889	6	405258	5	NULL	NULL	0	NULL	Z	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyacrylamide ( PAA ) - bentonite ( B ) and zeolite ( Z ) composites were prepared by direct polymerization of PAA in suspensions of B and Z. Phytate ( Phy ) immobilized onto the composites to obtain their Phy modifications .
	manualset3
125890	7	405258	5	NULL	NULL	0	NULL	Phytate ( Phy )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyacrylamide ( PAA ) - bentonite ( B ) and zeolite ( Z ) composites were prepared by direct polymerization of PAA in suspensions of B and Z. Phytate ( Phy ) immobilized onto the composites to obtain their Phy modifications .
	manualset3
125891	8	405258	5	NULL	NULL	0	NULL	composites 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyacrylamide ( PAA ) - bentonite ( B ) and zeolite ( Z ) composites were prepared by direct polymerization of PAA in suspensions of B and Z. Phytate ( Phy ) immobilized onto the composites to obtain their Phy modifications .
	manualset3
125892	9	405258	5	NULL	NULL	0	NULL	Phy modifications	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyacrylamide ( PAA ) - bentonite ( B ) and zeolite ( Z ) composites were prepared by direct polymerization of PAA in suspensions of B and Z. Phytate ( Phy ) immobilized onto the composites to obtain their Phy modifications .
	manualset3
125893	1	405259	5	NULL	NULL	0	NULL	Polyacrylamide gel electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyacrylamide gel electrophoresis of the purified alpha-L-fucosidase demonstrated the presence of six bands of protein which all contained fucosidase activity .
	manualset3
125894	2	405259	5	NULL	NULL	0	NULL	purified alpha-L-fucosidase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyacrylamide gel electrophoresis of the purified alpha-L-fucosidase demonstrated the presence of six bands of protein which all contained fucosidase activity .
	manualset3
125895	3	405259	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyacrylamide gel electrophoresis of the purified alpha-L-fucosidase demonstrated the presence of six bands of protein which all contained fucosidase activity .
	manualset3
125896	4	405259	5	NULL	NULL	0	NULL	six bands 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyacrylamide gel electrophoresis of the purified alpha-L-fucosidase demonstrated the presence of six bands of protein which all contained fucosidase activity .
	manualset3
125897	5	405259	5	NULL	NULL	0	NULL	protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyacrylamide gel electrophoresis of the purified alpha-L-fucosidase demonstrated the presence of six bands of protein which all contained fucosidase activity .
	manualset3
125898	6	405259	5	NULL	NULL	0	NULL	fucosidase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyacrylamide gel electrophoresis of the purified alpha-L-fucosidase demonstrated the presence of six bands of protein which all contained fucosidase activity .
	manualset3
125899	1	405260	5	NULL	NULL	0	NULL	Polyamine accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyamine accumulation and biosynthesis in a mouse L1210 leukemia .
	manualset3
125900	2	405260	5	NULL	NULL	0	NULL	biosynthesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyamine accumulation and biosynthesis in a mouse L1210 leukemia .
	manualset3
125901	3	405260	5	NULL	NULL	0	NULL	mouse L1210 leukemia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyamine accumulation and biosynthesis in a mouse L1210 leukemia .
	manualset3
125902	1	405261	5	NULL	NULL	0	NULL	Polybrominated diphenyl ethers ( PBDE )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Polybrominated diphenyl ethers ( PBDE ) are used as flame retardants in a wide variety of products .
	manualset3
125903	2	405261	5	NULL	NULL	0	NULL	flame retardants 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Polybrominated diphenyl ethers ( PBDE ) are used as flame retardants in a wide variety of products .
	manualset3
125904	3	405261	5	NULL	NULL	0	NULL	wide variety	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Polybrominated diphenyl ethers ( PBDE ) are used as flame retardants in a wide variety of products .
	manualset3
125905	4	405261	5	NULL	NULL	0	NULL	products 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Polybrominated diphenyl ethers ( PBDE ) are used as flame retardants in a wide variety of products .
	manualset3
125906	1	405262	5	NULL	NULL	0	NULL	history 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A history of stroke , gastrectomy , rheumatoid arthritis , steroid treatment , thyroid disease , alcohol abuse and anti-convulsant therapy was present in patients with femoral fracture but did not relate to any particular histomorphometric classification .
	manualset3
125907	2	405262	5	NULL	NULL	0	NULL	stroke 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A history of stroke , gastrectomy , rheumatoid arthritis , steroid treatment , thyroid disease , alcohol abuse and anti-convulsant therapy was present in patients with femoral fracture but did not relate to any particular histomorphometric classification .
	manualset3
125908	3	405262	5	NULL	NULL	0	NULL	gastrectomy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A history of stroke , gastrectomy , rheumatoid arthritis , steroid treatment , thyroid disease , alcohol abuse and anti-convulsant therapy was present in patients with femoral fracture but did not relate to any particular histomorphometric classification .
	manualset3
125909	4	405262	5	NULL	NULL	0	NULL	rheumatoid arthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A history of stroke , gastrectomy , rheumatoid arthritis , steroid treatment , thyroid disease , alcohol abuse and anti-convulsant therapy was present in patients with femoral fracture but did not relate to any particular histomorphometric classification .
	manualset3
125910	5	405262	5	NULL	NULL	0	NULL	steroid treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A history of stroke , gastrectomy , rheumatoid arthritis , steroid treatment , thyroid disease , alcohol abuse and anti-convulsant therapy was present in patients with femoral fracture but did not relate to any particular histomorphometric classification .
	manualset3
125911	6	405262	5	NULL	NULL	0	NULL	thyroid disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A history of stroke , gastrectomy , rheumatoid arthritis , steroid treatment , thyroid disease , alcohol abuse and anti-convulsant therapy was present in patients with femoral fracture but did not relate to any particular histomorphometric classification .
	manualset3
125912	7	405262	5	NULL	NULL	0	NULL	alcohol abuse 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A history of stroke , gastrectomy , rheumatoid arthritis , steroid treatment , thyroid disease , alcohol abuse and anti-convulsant therapy was present in patients with femoral fracture but did not relate to any particular histomorphometric classification .
	manualset3
125913	8	405262	5	NULL	NULL	0	NULL	anti-convulsant therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A history of stroke , gastrectomy , rheumatoid arthritis , steroid treatment , thyroid disease , alcohol abuse and anti-convulsant therapy was present in patients with femoral fracture but did not relate to any particular histomorphometric classification .
	manualset3
125914	9	405262	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A history of stroke , gastrectomy , rheumatoid arthritis , steroid treatment , thyroid disease , alcohol abuse and anti-convulsant therapy was present in patients with femoral fracture but did not relate to any particular histomorphometric classification .
	manualset3
125915	10	405262	5	NULL	NULL	0	NULL	femoral fracture 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A history of stroke , gastrectomy , rheumatoid arthritis , steroid treatment , thyroid disease , alcohol abuse and anti-convulsant therapy was present in patients with femoral fracture but did not relate to any particular histomorphometric classification .
	manualset3
125916	11	405262	5	NULL	NULL	0	NULL	histomorphometric classification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A history of stroke , gastrectomy , rheumatoid arthritis , steroid treatment , thyroid disease , alcohol abuse and anti-convulsant therapy was present in patients with femoral fracture but did not relate to any particular histomorphometric classification .
	manualset3
125917	1	405263	5	NULL	NULL	0	NULL	Polybrominated diphenyl ethers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Polybrominated diphenyl ethers in mudsnails ( Cipangopaludina cahayensis ) and sediments from an electronic waste recycling region in South China .
	manualset3
125918	2	405263	5	NULL	NULL	0	NULL	mudsnails ( Cipangopaludina cahayensis ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Polybrominated diphenyl ethers in mudsnails ( Cipangopaludina cahayensis ) and sediments from an electronic waste recycling region in South China .
	manualset3
125919	3	405263	5	NULL	NULL	0	NULL	sediments 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Polybrominated diphenyl ethers in mudsnails ( Cipangopaludina cahayensis ) and sediments from an electronic waste recycling region in South China .
	manualset3
125920	4	405263	5	NULL	NULL	0	NULL	electronic waste recycling region	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Polybrominated diphenyl ethers in mudsnails ( Cipangopaludina cahayensis ) and sediments from an electronic waste recycling region in South China .
	manualset3
125921	5	405263	5	NULL	NULL	0	NULL	South China	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Polybrominated diphenyl ethers in mudsnails ( Cipangopaludina cahayensis ) and sediments from an electronic waste recycling region in South China .
	manualset3
125922	1	405264	5	NULL	NULL	0	NULL	Polybutylcyanoacrylate nanoparticles	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Polybutylcyanoacrylate nanoparticles were prepared by an emulsion polymerization process .
	manualset3
125923	2	405264	5	NULL	NULL	0	NULL	emulsion polymerization process	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Polybutylcyanoacrylate nanoparticles were prepared by an emulsion polymerization process .
	manualset3
125924	1	405265	5	NULL	NULL	0	NULL	Polychlorinated biphenyl ( PCB ) congeners	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Polychlorinated biphenyl ( PCB ) congeners , a group of worldwide , persistent environmental contaminants , are known to cause carcinogenesis and tumor promotion , and may also affect the development of cancer metastasis .
	manualset3
125925	2	405265	5	NULL	NULL	0	NULL	group 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Polychlorinated biphenyl ( PCB ) congeners , a group of worldwide , persistent environmental contaminants , are known to cause carcinogenesis and tumor promotion , and may also affect the development of cancer metastasis .
	manualset3
125926	3	405265	5	NULL	NULL	0	NULL	persistent environmental contaminants	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Polychlorinated biphenyl ( PCB ) congeners , a group of worldwide , persistent environmental contaminants , are known to cause carcinogenesis and tumor promotion , and may also affect the development of cancer metastasis .
	manualset3
125928	5	405265	5	NULL	NULL	0	NULL	carcinogenesis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Polychlorinated biphenyl ( PCB ) congeners , a group of worldwide , persistent environmental contaminants , are known to cause carcinogenesis and tumor promotion , and may also affect the development of cancer metastasis .
	manualset3
125929	6	405265	5	NULL	NULL	0	NULL	tumor promotion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Polychlorinated biphenyl ( PCB ) congeners , a group of worldwide , persistent environmental contaminants , are known to cause carcinogenesis and tumor promotion , and may also affect the development of cancer metastasis .
	manualset3
125930	7	405265	5	NULL	NULL	0	NULL	development 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Polychlorinated biphenyl ( PCB ) congeners , a group of worldwide , persistent environmental contaminants , are known to cause carcinogenesis and tumor promotion , and may also affect the development of cancer metastasis .
	manualset3
125931	8	405265	5	NULL	NULL	0	NULL	cancer metastasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Polychlorinated biphenyl ( PCB ) congeners , a group of worldwide , persistent environmental contaminants , are known to cause carcinogenesis and tumor promotion , and may also affect the development of cancer metastasis .
	manualset3
125932	1	405266	5	NULL	NULL	0	NULL	Polyethylene tubing	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyethylene and polypropylene tubing absorb significantly less volatile anesthetic than conductive rubber ; however , this is not the case with polyvinyl chloride tubing .
	manualset3
125933	2	405266	5	NULL	NULL	0	NULL	polypropylene tubing	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyethylene and polypropylene tubing absorb significantly less volatile anesthetic than conductive rubber ; however , this is not the case with polyvinyl chloride tubing .
	manualset3
125934	3	405266	5	NULL	NULL	0	NULL	less volatile anesthetic 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyethylene and polypropylene tubing absorb significantly less volatile anesthetic than conductive rubber ; however , this is not the case with polyvinyl chloride tubing .
	manualset3
125935	4	405266	5	NULL	NULL	0	NULL	conductive rubber	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyethylene and polypropylene tubing absorb significantly less volatile anesthetic than conductive rubber ; however , this is not the case with polyvinyl chloride tubing .
	manualset3
125936	5	405266	5	NULL	NULL	0	NULL	case	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyethylene and polypropylene tubing absorb significantly less volatile anesthetic than conductive rubber ; however , this is not the case with polyvinyl chloride tubing .
	manualset3
125937	6	405266	5	NULL	NULL	0	NULL	polyvinyl chloride tubing	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyethylene and polypropylene tubing absorb significantly less volatile anesthetic than conductive rubber ; however , this is not the case with polyvinyl chloride tubing .
	manualset3
126100	1	405267	5	NULL	NULL	0	NULL	Polymer-based controlled-release technology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymer-based controlled-release technology has enabled us to demonstrate : that the controlled release of insulin from polymer matrices can indeed be used to control diabetes mellitus but does so at the expense of hyperinsulinemia and hypoglycemia ; and that somatostatin can be delivered in similar fashion , so as to provide glucose homeostasis in a more physiologic range , at lower insulin levels and at somatostatin doses below those used in intermittent infusion studies ; and , that microgram quantities of a drug can be delivered successfully in vivo with intact biological function and in a manner that can be monitored continuously .
	manualset3
126102	3	405267	5	NULL	NULL	0	NULL	release	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymer-based controlled-release technology has enabled us to demonstrate : that the controlled release of insulin from polymer matrices can indeed be used to control diabetes mellitus but does so at the expense of hyperinsulinemia and hypoglycemia ; and that somatostatin can be delivered in similar fashion , so as to provide glucose homeostasis in a more physiologic range , at lower insulin levels and at somatostatin doses below those used in intermittent infusion studies ; and , that microgram quantities of a drug can be delivered successfully in vivo with intact biological function and in a manner that can be monitored continuously .
	manualset3
126103	4	405267	5	NULL	NULL	0	NULL	insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymer-based controlled-release technology has enabled us to demonstrate : that the controlled release of insulin from polymer matrices can indeed be used to control diabetes mellitus but does so at the expense of hyperinsulinemia and hypoglycemia ; and that somatostatin can be delivered in similar fashion , so as to provide glucose homeostasis in a more physiologic range , at lower insulin levels and at somatostatin doses below those used in intermittent infusion studies ; and , that microgram quantities of a drug can be delivered successfully in vivo with intact biological function and in a manner that can be monitored continuously .
	manualset3
126104	5	405267	5	NULL	NULL	0	NULL	polymer matrices	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymer-based controlled-release technology has enabled us to demonstrate : that the controlled release of insulin from polymer matrices can indeed be used to control diabetes mellitus but does so at the expense of hyperinsulinemia and hypoglycemia ; and that somatostatin can be delivered in similar fashion , so as to provide glucose homeostasis in a more physiologic range , at lower insulin levels and at somatostatin doses below those used in intermittent infusion studies ; and , that microgram quantities of a drug can be delivered successfully in vivo with intact biological function and in a manner that can be monitored continuously .
	manualset3
126106	7	405267	5	NULL	NULL	0	NULL	diabetes mellitus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymer-based controlled-release technology has enabled us to demonstrate : that the controlled release of insulin from polymer matrices can indeed be used to control diabetes mellitus but does so at the expense of hyperinsulinemia and hypoglycemia ; and that somatostatin can be delivered in similar fashion , so as to provide glucose homeostasis in a more physiologic range , at lower insulin levels and at somatostatin doses below those used in intermittent infusion studies ; and , that microgram quantities of a drug can be delivered successfully in vivo with intact biological function and in a manner that can be monitored continuously .
	manualset3
126109	8	405267	5	NULL	NULL	0	NULL	expense	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymer-based controlled-release technology has enabled us to demonstrate : that the controlled release of insulin from polymer matrices can indeed be used to control diabetes mellitus but does so at the expense of hyperinsulinemia and hypoglycemia ; and that somatostatin can be delivered in similar fashion , so as to provide glucose homeostasis in a more physiologic range , at lower insulin levels and at somatostatin doses below those used in intermittent infusion studies ; and , that microgram quantities of a drug can be delivered successfully in vivo with intact biological function and in a manner that can be monitored continuously .
	manualset3
126110	9	405267	5	NULL	NULL	0	NULL	hyperinsulinemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymer-based controlled-release technology has enabled us to demonstrate : that the controlled release of insulin from polymer matrices can indeed be used to control diabetes mellitus but does so at the expense of hyperinsulinemia and hypoglycemia ; and that somatostatin can be delivered in similar fashion , so as to provide glucose homeostasis in a more physiologic range , at lower insulin levels and at somatostatin doses below those used in intermittent infusion studies ; and , that microgram quantities of a drug can be delivered successfully in vivo with intact biological function and in a manner that can be monitored continuously .
	manualset3
126111	10	405267	5	NULL	NULL	0	NULL	hypoglycemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymer-based controlled-release technology has enabled us to demonstrate : that the controlled release of insulin from polymer matrices can indeed be used to control diabetes mellitus but does so at the expense of hyperinsulinemia and hypoglycemia ; and that somatostatin can be delivered in similar fashion , so as to provide glucose homeostasis in a more physiologic range , at lower insulin levels and at somatostatin doses below those used in intermittent infusion studies ; and , that microgram quantities of a drug can be delivered successfully in vivo with intact biological function and in a manner that can be monitored continuously .
	manualset3
126114	11	405267	5	NULL	NULL	0	NULL	somatostatin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymer-based controlled-release technology has enabled us to demonstrate : that the controlled release of insulin from polymer matrices can indeed be used to control diabetes mellitus but does so at the expense of hyperinsulinemia and hypoglycemia ; and that somatostatin can be delivered in similar fashion , so as to provide glucose homeostasis in a more physiologic range , at lower insulin levels and at somatostatin doses below those used in intermittent infusion studies ; and , that microgram quantities of a drug can be delivered successfully in vivo with intact biological function and in a manner that can be monitored continuously .
	manualset3
126117	12	405267	5	NULL	NULL	0	NULL	glucose homeostasis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymer-based controlled-release technology has enabled us to demonstrate : that the controlled release of insulin from polymer matrices can indeed be used to control diabetes mellitus but does so at the expense of hyperinsulinemia and hypoglycemia ; and that somatostatin can be delivered in similar fashion , so as to provide glucose homeostasis in a more physiologic range , at lower insulin levels and at somatostatin doses below those used in intermittent infusion studies ; and , that microgram quantities of a drug can be delivered successfully in vivo with intact biological function and in a manner that can be monitored continuously .
	manualset3
126119	13	405267	5	NULL	NULL	0	NULL	physiologic range	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymer-based controlled-release technology has enabled us to demonstrate : that the controlled release of insulin from polymer matrices can indeed be used to control diabetes mellitus but does so at the expense of hyperinsulinemia and hypoglycemia ; and that somatostatin can be delivered in similar fashion , so as to provide glucose homeostasis in a more physiologic range , at lower insulin levels and at somatostatin doses below those used in intermittent infusion studies ; and , that microgram quantities of a drug can be delivered successfully in vivo with intact biological function and in a manner that can be monitored continuously .
	manualset3
126124	14	405267	5	NULL	NULL	0	NULL	lower insulin levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymer-based controlled-release technology has enabled us to demonstrate : that the controlled release of insulin from polymer matrices can indeed be used to control diabetes mellitus but does so at the expense of hyperinsulinemia and hypoglycemia ; and that somatostatin can be delivered in similar fashion , so as to provide glucose homeostasis in a more physiologic range , at lower insulin levels and at somatostatin doses below those used in intermittent infusion studies ; and , that microgram quantities of a drug can be delivered successfully in vivo with intact biological function and in a manner that can be monitored continuously .
	manualset3
126127	15	405267	5	NULL	NULL	0	NULL	somatostatin doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymer-based controlled-release technology has enabled us to demonstrate : that the controlled release of insulin from polymer matrices can indeed be used to control diabetes mellitus but does so at the expense of hyperinsulinemia and hypoglycemia ; and that somatostatin can be delivered in similar fashion , so as to provide glucose homeostasis in a more physiologic range , at lower insulin levels and at somatostatin doses below those used in intermittent infusion studies ; and , that microgram quantities of a drug can be delivered successfully in vivo with intact biological function and in a manner that can be monitored continuously .
	manualset3
126128	16	405267	5	NULL	NULL	0	NULL	intermittent infusion studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymer-based controlled-release technology has enabled us to demonstrate : that the controlled release of insulin from polymer matrices can indeed be used to control diabetes mellitus but does so at the expense of hyperinsulinemia and hypoglycemia ; and that somatostatin can be delivered in similar fashion , so as to provide glucose homeostasis in a more physiologic range , at lower insulin levels and at somatostatin doses below those used in intermittent infusion studies ; and , that microgram quantities of a drug can be delivered successfully in vivo with intact biological function and in a manner that can be monitored continuously .
	manualset3
126129	17	405267	5	NULL	NULL	0	NULL	microgram quantities	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymer-based controlled-release technology has enabled us to demonstrate : that the controlled release of insulin from polymer matrices can indeed be used to control diabetes mellitus but does so at the expense of hyperinsulinemia and hypoglycemia ; and that somatostatin can be delivered in similar fashion , so as to provide glucose homeostasis in a more physiologic range , at lower insulin levels and at somatostatin doses below those used in intermittent infusion studies ; and , that microgram quantities of a drug can be delivered successfully in vivo with intact biological function and in a manner that can be monitored continuously .
	manualset3
126131	18	405267	5	NULL	NULL	0	NULL	drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymer-based controlled-release technology has enabled us to demonstrate : that the controlled release of insulin from polymer matrices can indeed be used to control diabetes mellitus but does so at the expense of hyperinsulinemia and hypoglycemia ; and that somatostatin can be delivered in similar fashion , so as to provide glucose homeostasis in a more physiologic range , at lower insulin levels and at somatostatin doses below those used in intermittent infusion studies ; and , that microgram quantities of a drug can be delivered successfully in vivo with intact biological function and in a manner that can be monitored continuously .
	manualset3
126134	19	405267	5	NULL	NULL	0	NULL	biological function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymer-based controlled-release technology has enabled us to demonstrate : that the controlled release of insulin from polymer matrices can indeed be used to control diabetes mellitus but does so at the expense of hyperinsulinemia and hypoglycemia ; and that somatostatin can be delivered in similar fashion , so as to provide glucose homeostasis in a more physiologic range , at lower insulin levels and at somatostatin doses below those used in intermittent infusion studies ; and , that microgram quantities of a drug can be delivered successfully in vivo with intact biological function and in a manner that can be monitored continuously .
	manualset3
126135	1	405268	5	NULL	NULL	0	NULL	Polymerase chain reaction analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymerase chain reaction analysis of mRNA extracted from these cells indicated they contained mRNA for B7 , a known counter receptor for CTLA4 and CD28 .
	manualset3
126136	2	405268	5	NULL	NULL	0	NULL	mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymerase chain reaction analysis of mRNA extracted from these cells indicated they contained mRNA for B7 , a known counter receptor for CTLA4 and CD28 .
	manualset3
126138	3	405268	5	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymerase chain reaction analysis of mRNA extracted from these cells indicated they contained mRNA for B7 , a known counter receptor for CTLA4 and CD28 .
	manualset3
126140	4	405268	5	NULL	NULL	0	NULL	mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymerase chain reaction analysis of mRNA extracted from these cells indicated they contained mRNA for B7 , a known counter receptor for CTLA4 and CD28 .
	manualset3
126143	5	405268	5	NULL	NULL	0	NULL	B7 , a known counter receptor for CTLA4 and CD28	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymerase chain reaction analysis of mRNA extracted from these cells indicated they contained mRNA for B7 , a known counter receptor for CTLA4 and CD28 .
	manualset3
126144	1	405269	5	NULL	NULL	0	NULL	Polymerase chain reaction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymerase chain reaction was used first to amplify a part of the chlamydial genome that included the leader sequence and all four variable domains of the major outer membrane protein ( MOMP ) of the 15 serovars of C. trachomatis .
	manualset3
126146	3	405269	5	NULL	NULL	0	NULL	chlamydial genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymerase chain reaction was used first to amplify a part of the chlamydial genome that included the leader sequence and all four variable domains of the major outer membrane protein ( MOMP ) of the 15 serovars of C. trachomatis .
	manualset3
126147	4	405269	5	NULL	NULL	0	NULL	leader sequence 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymerase chain reaction was used first to amplify a part of the chlamydial genome that included the leader sequence and all four variable domains of the major outer membrane protein ( MOMP ) of the 15 serovars of C. trachomatis .
	manualset3
126148	5	405269	5	NULL	NULL	0	NULL	four	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymerase chain reaction was used first to amplify a part of the chlamydial genome that included the leader sequence and all four variable domains of the major outer membrane protein ( MOMP ) of the 15 serovars of C. trachomatis .
	manualset3
126149	6	405269	5	NULL	NULL	0	NULL	variable domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymerase chain reaction was used first to amplify a part of the chlamydial genome that included the leader sequence and all four variable domains of the major outer membrane protein ( MOMP ) of the 15 serovars of C. trachomatis .
	manualset3
126150	7	405269	5	NULL	NULL	0	NULL	major outer membrane protein ( MOMP ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymerase chain reaction was used first to amplify a part of the chlamydial genome that included the leader sequence and all four variable domains of the major outer membrane protein ( MOMP ) of the 15 serovars of C. trachomatis .
	manualset3
126151	8	405269	5	NULL	NULL	0	NULL	15 serovars 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymerase chain reaction was used first to amplify a part of the chlamydial genome that included the leader sequence and all four variable domains of the major outer membrane protein ( MOMP ) of the 15 serovars of C. trachomatis .
	manualset3
126152	9	405269	5	NULL	NULL	0	NULL	C. trachomatis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymerase chain reaction was used first to amplify a part of the chlamydial genome that included the leader sequence and all four variable domains of the major outer membrane protein ( MOMP ) of the 15 serovars of C. trachomatis .
	manualset3
126153	1	405270	5	NULL	NULL	0	NULL	Polymeric biomaterials	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymeric biomaterials have played an integral role in tissue engineering , biomedical devices , and targeted drug delivery .
	manualset3
126154	2	405270	5	NULL	NULL	0	NULL	integral role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymeric biomaterials have played an integral role in tissue engineering , biomedical devices , and targeted drug delivery .
	manualset3
126155	3	405270	5	NULL	NULL	0	NULL	tissue engineering	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymeric biomaterials have played an integral role in tissue engineering , biomedical devices , and targeted drug delivery .
	manualset3
126156	4	405270	5	NULL	NULL	0	NULL	biomedical devices	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymeric biomaterials have played an integral role in tissue engineering , biomedical devices , and targeted drug delivery .
	manualset3
126157	5	405270	5	NULL	NULL	0	NULL	 targeted drug delivery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymeric biomaterials have played an integral role in tissue engineering , biomedical devices , and targeted drug delivery .
	manualset3
126158	1	405271	5	NULL	NULL	0	NULL	Polymorphic Alu insertions	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphic Alu insertions in six Brazilian African-derived populations .
	manualset3
126159	2	405271	5	NULL	NULL	0	NULL	six	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphic Alu insertions in six Brazilian African-derived populations .
	manualset3
126161	3	405271	5	NULL	NULL	0	NULL	Brazilian African-derived populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphic Alu insertions in six Brazilian African-derived populations .
	manualset3
126162	1	405272	5	NULL	NULL	0	NULL	Polymorphic ventricular tachycardia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphic ventricular tachycardia in acute myocardial infarction treated by thrombolysis : reperfusion , complication or iatrogenic sign ?
	manualset3
126163	2	405272	5	NULL	NULL	0	NULL	acute myocardial infarction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphic ventricular tachycardia in acute myocardial infarction treated by thrombolysis : reperfusion , complication or iatrogenic sign ?
	manualset3
126164	3	405272	5	NULL	NULL	0	NULL	thrombolysis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphic ventricular tachycardia in acute myocardial infarction treated by thrombolysis : reperfusion , complication or iatrogenic sign ?
	manualset3
126165	4	405272	5	NULL	NULL	0	NULL	reperfusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphic ventricular tachycardia in acute myocardial infarction treated by thrombolysis : reperfusion , complication or iatrogenic sign ?
	manualset3
126166	5	405272	5	NULL	NULL	0	NULL	complication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphic ventricular tachycardia in acute myocardial infarction treated by thrombolysis : reperfusion , complication or iatrogenic sign ?
	manualset3
126167	6	405272	5	NULL	NULL	0	NULL	iatrogenic sign	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphic ventricular tachycardia in acute myocardial infarction treated by thrombolysis : reperfusion , complication or iatrogenic sign ?
	manualset3
126221	1	405273	5	NULL	NULL	0	NULL	Polymorphism G80A	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphism G80A in the reduced folate carrier gene and its relationship to methotrexate plasma levels and outcome of childhood acute lymphoblastic leukemia .
	manualset3
126222	2	405273	5	NULL	NULL	0	NULL	folate carrier gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphism G80A in the reduced folate carrier gene and its relationship to methotrexate plasma levels and outcome of childhood acute lymphoblastic leukemia .
	manualset3
126223	3	405273	5	NULL	NULL	0	NULL	relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphism G80A in the reduced folate carrier gene and its relationship to methotrexate plasma levels and outcome of childhood acute lymphoblastic leukemia .
	manualset3
126224	4	405273	5	NULL	NULL	0	NULL	methotrexate plasma levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphism G80A in the reduced folate carrier gene and its relationship to methotrexate plasma levels and outcome of childhood acute lymphoblastic leukemia .
	manualset3
126225	5	405273	5	NULL	NULL	0	NULL	outcome 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphism G80A in the reduced folate carrier gene and its relationship to methotrexate plasma levels and outcome of childhood acute lymphoblastic leukemia .
	manualset3
126226	6	405273	5	NULL	NULL	0	NULL	childhood acute lymphoblastic leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphism G80A in the reduced folate carrier gene and its relationship to methotrexate plasma levels and outcome of childhood acute lymphoblastic leukemia .
	manualset3
126227	1	405274	5	NULL	NULL	0	NULL	Polymorphism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphism and distribution of HLA-DR2 alleles in Mexican populations .
	manualset3
126228	2	405274	5	NULL	NULL	0	NULL	distribution 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphism and distribution of HLA-DR2 alleles in Mexican populations .
	manualset3
126229	3	405274	5	NULL	NULL	0	NULL	 HLA-DR2 alleles 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphism and distribution of HLA-DR2 alleles in Mexican populations .
	manualset3
126230	4	405274	5	NULL	NULL	0	NULL	Mexican populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphism and distribution of HLA-DR2 alleles in Mexican populations .
	manualset3
126231	1	405275	5	NULL	NULL	0	NULL	Polymorphism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphism in jasmonate signaling partially accounts for the variety of volatiles produced by Nicotiana attenuata plants in a native population .
	manualset3
126232	2	405275	5	NULL	NULL	0	NULL	jasmonate signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphism in jasmonate signaling partially accounts for the variety of volatiles produced by Nicotiana attenuata plants in a native population .
	manualset3
126233	3	405275	5	NULL	NULL	0	NULL	variety 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphism in jasmonate signaling partially accounts for the variety of volatiles produced by Nicotiana attenuata plants in a native population .
	manualset3
126234	4	405275	5	NULL	NULL	0	NULL	volatiles 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphism in jasmonate signaling partially accounts for the variety of volatiles produced by Nicotiana attenuata plants in a native population .
	manualset3
126235	5	405275	5	NULL	NULL	0	NULL	Nicotiana attenuata plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphism in jasmonate signaling partially accounts for the variety of volatiles produced by Nicotiana attenuata plants in a native population .
	manualset3
126236	6	405275	5	NULL	NULL	NULL	NULL	native population	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Polymorphism in jasmonate signaling partially accounts for the variety of volatiles produced by Nicotiana attenuata plants in a native population .
	manualset3
126237	1	405276	5	NULL	NULL	0	NULL	Polymorphism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphism of the 5-HTT gene promoter was only partly responsible for the increased 5-HTT expression in PH , because PA-SMCs from patients exhibited higher 5-HTT levels than same-genotype cells from controls and no additional promoter sequence alterations were found .
	manualset3
126238	2	405276	5	NULL	NULL	0	NULL	5-HTT gene promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphism of the 5-HTT gene promoter was only partly responsible for the increased 5-HTT expression in PH , because PA-SMCs from patients exhibited higher 5-HTT levels than same-genotype cells from controls and no additional promoter sequence alterations were found .
	manualset3
126239	3	405276	5	NULL	NULL	0	NULL	5-HTT expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphism of the 5-HTT gene promoter was only partly responsible for the increased 5-HTT expression in PH , because PA-SMCs from patients exhibited higher 5-HTT levels than same-genotype cells from controls and no additional promoter sequence alterations were found .
	manualset3
126240	4	405276	5	NULL	NULL	0	NULL	PH	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphism of the 5-HTT gene promoter was only partly responsible for the increased 5-HTT expression in PH , because PA-SMCs from patients exhibited higher 5-HTT levels than same-genotype cells from controls and no additional promoter sequence alterations were found .
	manualset3
126241	5	405276	5	NULL	NULL	0	NULL	PA-SMCs 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphism of the 5-HTT gene promoter was only partly responsible for the increased 5-HTT expression in PH , because PA-SMCs from patients exhibited higher 5-HTT levels than same-genotype cells from controls and no additional promoter sequence alterations were found .
	manualset3
126242	6	405276	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphism of the 5-HTT gene promoter was only partly responsible for the increased 5-HTT expression in PH , because PA-SMCs from patients exhibited higher 5-HTT levels than same-genotype cells from controls and no additional promoter sequence alterations were found .
	manualset3
126243	7	405276	5	NULL	NULL	0	NULL	5-HTT levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphism of the 5-HTT gene promoter was only partly responsible for the increased 5-HTT expression in PH , because PA-SMCs from patients exhibited higher 5-HTT levels than same-genotype cells from controls and no additional promoter sequence alterations were found .
	manualset3
126244	8	405276	5	NULL	NULL	0	NULL	same-genotype cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphism of the 5-HTT gene promoter was only partly responsible for the increased 5-HTT expression in PH , because PA-SMCs from patients exhibited higher 5-HTT levels than same-genotype cells from controls and no additional promoter sequence alterations were found .
	manualset3
126245	9	405276	5	NULL	NULL	0	NULL	controls 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphism of the 5-HTT gene promoter was only partly responsible for the increased 5-HTT expression in PH , because PA-SMCs from patients exhibited higher 5-HTT levels than same-genotype cells from controls and no additional promoter sequence alterations were found .
	manualset3
126246	10	405276	5	NULL	NULL	0	NULL	promoter sequence alterations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphism of the 5-HTT gene promoter was only partly responsible for the increased 5-HTT expression in PH , because PA-SMCs from patients exhibited higher 5-HTT levels than same-genotype cells from controls and no additional promoter sequence alterations were found .
	manualset3
126247	1	405277	5	NULL	NULL	0	NULL	Polymorphisms 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphisms and reconstructed haplotypes of FADS1 and the upstream region of FADS2 showed strong associations with levels of the n-6 LC-PUFA arachidonic acid ( 20 : 4 n-6 ) .
	manualset3
126248	2	405277	5	NULL	NULL	0	NULL	reconstructed haplotypes of FADS1	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphisms and reconstructed haplotypes of FADS1 and the upstream region of FADS2 showed strong associations with levels of the n-6 LC-PUFA arachidonic acid ( 20 : 4 n-6 ) .
	manualset3
126249	3	405277	5	NULL	NULL	0	NULL	upstream region of FADS2	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphisms and reconstructed haplotypes of FADS1 and the upstream region of FADS2 showed strong associations with levels of the n-6 LC-PUFA arachidonic acid ( 20 : 4 n-6 ) .
	manualset3
126250	4	405277	5	NULL	NULL	NULL	NULL	strong associations	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Polymorphisms and reconstructed haplotypes of FADS1 and the upstream region of FADS2 showed strong associations with levels of the n-6 LC-PUFA arachidonic acid ( 20 : 4 n-6 ) .
	manualset3
126251	5	405277	5	NULL	NULL	0	NULL	levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphisms and reconstructed haplotypes of FADS1 and the upstream region of FADS2 showed strong associations with levels of the n-6 LC-PUFA arachidonic acid ( 20 : 4 n-6 ) .
	manualset3
126252	6	405277	5	NULL	NULL	0	NULL	n-6 LC-PUFA arachidonic acid	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphisms and reconstructed haplotypes of FADS1 and the upstream region of FADS2 showed strong associations with levels of the n-6 LC-PUFA arachidonic acid ( 20 : 4 n-6 ) .
	manualset3
126253	7	405277	5	NULL	NULL	0	NULL	20 : 4 n-6	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphisms and reconstructed haplotypes of FADS1 and the upstream region of FADS2 showed strong associations with levels of the n-6 LC-PUFA arachidonic acid ( 20 : 4 n-6 ) .
	manualset3
126254	1	405278	5	NULL	NULL	0	NULL	Polymorphisms 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphisms in folate pathway genes may influence the susceptibility to acute lymphoblastic leukemia ( ALL ) .
	manualset3
126255	2	405278	5	NULL	NULL	0	NULL	folate pathway genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphisms in folate pathway genes may influence the susceptibility to acute lymphoblastic leukemia ( ALL ) .
	manualset3
126256	3	405278	5	NULL	NULL	0	NULL	susceptibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphisms in folate pathway genes may influence the susceptibility to acute lymphoblastic leukemia ( ALL ) .
	manualset3
126257	4	405278	5	NULL	NULL	0	NULL	acute lymphoblastic leukemia ( ALL )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphisms in folate pathway genes may influence the susceptibility to acute lymphoblastic leukemia ( ALL ) .
	manualset3
126258	1	405279	5	NULL	NULL	0	NULL	( Ca ( 2 + ) ) ( i )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	( Ca ( 2 + ) ) ( i ) was measured in microdissected arterioles using ratiometric photometry of fura 2 fluorescence .
	manualset3
126259	2	405279	5	NULL	NULL	0	NULL	microdissected arterioles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Ca ( 2 + ) ) ( i ) was measured in microdissected arterioles using ratiometric photometry of fura 2 fluorescence .
	manualset3
126260	3	405279	5	NULL	NULL	0	NULL	ratiometric photometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Ca ( 2 + ) ) ( i ) was measured in microdissected arterioles using ratiometric photometry of fura 2 fluorescence .
	manualset3
126261	4	405279	5	NULL	NULL	0	NULL	fura 2 fluorescence	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	( Ca ( 2 + ) ) ( i ) was measured in microdissected arterioles using ratiometric photometry of fura 2 fluorescence .
	manualset3
126262	1	405280	5	NULL	NULL	0	NULL	hot-film anemometer system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A hot-film anemometer system has been calibrated and evaluated for the measurement of sinusoidal water motions used in stimulating the mechanosensory lateral line system of a teleost fish .
	manualset3
126263	2	405280	5	NULL	NULL	0	NULL	measurement 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A hot-film anemometer system has been calibrated and evaluated for the measurement of sinusoidal water motions used in stimulating the mechanosensory lateral line system of a teleost fish .
	manualset3
126264	3	405280	5	NULL	NULL	0	NULL	sinusoidal water motions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A hot-film anemometer system has been calibrated and evaluated for the measurement of sinusoidal water motions used in stimulating the mechanosensory lateral line system of a teleost fish .
	manualset3
126265	4	405280	5	NULL	NULL	0	NULL	mechanosensory lateral line system	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A hot-film anemometer system has been calibrated and evaluated for the measurement of sinusoidal water motions used in stimulating the mechanosensory lateral line system of a teleost fish .
	manualset3
126266	5	405280	5	NULL	NULL	0	NULL	teleost fish	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A hot-film anemometer system has been calibrated and evaluated for the measurement of sinusoidal water motions used in stimulating the mechanosensory lateral line system of a teleost fish .
	manualset3
126267	1	405281	5	NULL	NULL	0	NULL	Polymorphonuclear neutrophils ( PMNs )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphonuclear neutrophils ( PMNs ) , which have been detected in the earliest stages of atherosclerotic lesions , are one of the most likely sources of the reactive oxygen species that cause such stress .
	manualset3
126268	2	405281	5	NULL	NULL	0	NULL	earliest stages	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphonuclear neutrophils ( PMNs ) , which have been detected in the earliest stages of atherosclerotic lesions , are one of the most likely sources of the reactive oxygen species that cause such stress .
	manualset3
126269	3	405281	5	NULL	NULL	0	NULL	atherosclerotic lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphonuclear neutrophils ( PMNs ) , which have been detected in the earliest stages of atherosclerotic lesions , are one of the most likely sources of the reactive oxygen species that cause such stress .
	manualset3
126270	4	405281	5	NULL	NULL	0	NULL	one 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphonuclear neutrophils ( PMNs ) , which have been detected in the earliest stages of atherosclerotic lesions , are one of the most likely sources of the reactive oxygen species that cause such stress .
	manualset3
126271	5	405281	5	NULL	NULL	0	NULL	sources 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphonuclear neutrophils ( PMNs ) , which have been detected in the earliest stages of atherosclerotic lesions , are one of the most likely sources of the reactive oxygen species that cause such stress .
	manualset3
126272	6	405281	5	NULL	NULL	0	NULL	reactive oxygen species	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Polymorphonuclear neutrophils ( PMNs ) , which have been detected in the earliest stages of atherosclerotic lesions , are one of the most likely sources of the reactive oxygen species that cause such stress .
	manualset3
126274	7	405281	5	NULL	NULL	NULL	NULL	stress 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Polymorphonuclear neutrophils ( PMNs ) , which have been detected in the earliest stages of atherosclerotic lesions , are one of the most likely sources of the reactive oxygen species that cause such stress .
	manualset3
126275	1	405282	5	NULL	NULL	0	NULL	Polyol species	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyol species in cerebrospinal fluid and plasma -- ribitol , arabitol , xylitol , 1 , 5-anhydrosorbitol , myo-inositol , mannitol , sorbitol , and galactitol -- simultaneously were quantitated by a capillary gas chromatography/ion trap ( mass spectrometric ) detection method .
	manualset3
126276	2	405282	5	NULL	NULL	0	NULL	cerebrospinal fluid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyol species in cerebrospinal fluid and plasma -- ribitol , arabitol , xylitol , 1 , 5-anhydrosorbitol , myo-inositol , mannitol , sorbitol , and galactitol -- simultaneously were quantitated by a capillary gas chromatography/ion trap ( mass spectrometric ) detection method .
	manualset3
126277	3	405282	5	NULL	NULL	0	NULL	plasma 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyol species in cerebrospinal fluid and plasma -- ribitol , arabitol , xylitol , 1 , 5-anhydrosorbitol , myo-inositol , mannitol , sorbitol , and galactitol -- simultaneously were quantitated by a capillary gas chromatography/ion trap ( mass spectrometric ) detection method .
	manualset3
126278	4	405282	5	NULL	NULL	0	NULL	ribitol 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyol species in cerebrospinal fluid and plasma -- ribitol , arabitol , xylitol , 1 , 5-anhydrosorbitol , myo-inositol , mannitol , sorbitol , and galactitol -- simultaneously were quantitated by a capillary gas chromatography/ion trap ( mass spectrometric ) detection method .
	manualset3
126279	5	405282	5	NULL	NULL	0	NULL	arabitol 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyol species in cerebrospinal fluid and plasma -- ribitol , arabitol , xylitol , 1 , 5-anhydrosorbitol , myo-inositol , mannitol , sorbitol , and galactitol -- simultaneously were quantitated by a capillary gas chromatography/ion trap ( mass spectrometric ) detection method .
	manualset3
126280	6	405282	5	NULL	NULL	0	NULL	xylitol 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyol species in cerebrospinal fluid and plasma -- ribitol , arabitol , xylitol , 1 , 5-anhydrosorbitol , myo-inositol , mannitol , sorbitol , and galactitol -- simultaneously were quantitated by a capillary gas chromatography/ion trap ( mass spectrometric ) detection method .
	manualset3
126281	7	405282	5	NULL	NULL	0	NULL	1 , 5-anhydrosorbitol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyol species in cerebrospinal fluid and plasma -- ribitol , arabitol , xylitol , 1 , 5-anhydrosorbitol , myo-inositol , mannitol , sorbitol , and galactitol -- simultaneously were quantitated by a capillary gas chromatography/ion trap ( mass spectrometric ) detection method .
	manualset3
126282	8	405282	5	NULL	NULL	0	NULL	myo-inositol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyol species in cerebrospinal fluid and plasma -- ribitol , arabitol , xylitol , 1 , 5-anhydrosorbitol , myo-inositol , mannitol , sorbitol , and galactitol -- simultaneously were quantitated by a capillary gas chromatography/ion trap ( mass spectrometric ) detection method .
	manualset3
126283	9	405282	5	NULL	NULL	0	NULL	mannitol 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyol species in cerebrospinal fluid and plasma -- ribitol , arabitol , xylitol , 1 , 5-anhydrosorbitol , myo-inositol , mannitol , sorbitol , and galactitol -- simultaneously were quantitated by a capillary gas chromatography/ion trap ( mass spectrometric ) detection method .
	manualset3
126284	10	405282	5	NULL	NULL	0	NULL	sorbitol 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyol species in cerebrospinal fluid and plasma -- ribitol , arabitol , xylitol , 1 , 5-anhydrosorbitol , myo-inositol , mannitol , sorbitol , and galactitol -- simultaneously were quantitated by a capillary gas chromatography/ion trap ( mass spectrometric ) detection method .
	manualset3
126285	11	405282	5	NULL	NULL	0	NULL	galactitol 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyol species in cerebrospinal fluid and plasma -- ribitol , arabitol , xylitol , 1 , 5-anhydrosorbitol , myo-inositol , mannitol , sorbitol , and galactitol -- simultaneously were quantitated by a capillary gas chromatography/ion trap ( mass spectrometric ) detection method .
	manualset3
126286	12	405282	5	NULL	NULL	0	NULL	capillary gas chromatography/ion trap ( mass spectrometric ) detection method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyol species in cerebrospinal fluid and plasma -- ribitol , arabitol , xylitol , 1 , 5-anhydrosorbitol , myo-inositol , mannitol , sorbitol , and galactitol -- simultaneously were quantitated by a capillary gas chromatography/ion trap ( mass spectrometric ) detection method .
	manualset3
126287	1	405283	5	NULL	NULL	0	NULL	Polypeptides 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Polypeptides that define a protein family termed RGS ( for regulators of G-protein signalling ) are encoded by the SST2 gene of the yeast Saccharomyces cerevisiae , the EGL-10 gene of the nematode Caenorhabdatis elegans , and several related mammalian genes .
	manualset3
126288	2	405283	5	NULL	NULL	0	NULL	protein family 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Polypeptides that define a protein family termed RGS ( for regulators of G-protein signalling ) are encoded by the SST2 gene of the yeast Saccharomyces cerevisiae , the EGL-10 gene of the nematode Caenorhabdatis elegans , and several related mammalian genes .
	manualset3
126289	3	405283	5	NULL	NULL	0	NULL	RGS ( for regulators of G-protein signalling )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Polypeptides that define a protein family termed RGS ( for regulators of G-protein signalling ) are encoded by the SST2 gene of the yeast Saccharomyces cerevisiae , the EGL-10 gene of the nematode Caenorhabdatis elegans , and several related mammalian genes .
	manualset3
126290	4	405283	5	NULL	NULL	0	NULL	SST2 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Polypeptides that define a protein family termed RGS ( for regulators of G-protein signalling ) are encoded by the SST2 gene of the yeast Saccharomyces cerevisiae , the EGL-10 gene of the nematode Caenorhabdatis elegans , and several related mammalian genes .
	manualset3
126291	5	405283	5	NULL	NULL	0	NULL	yeast Saccharomyces cerevisiae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Polypeptides that define a protein family termed RGS ( for regulators of G-protein signalling ) are encoded by the SST2 gene of the yeast Saccharomyces cerevisiae , the EGL-10 gene of the nematode Caenorhabdatis elegans , and several related mammalian genes .
	manualset3
126292	6	405283	5	NULL	NULL	0	NULL	EGL-10 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Polypeptides that define a protein family termed RGS ( for regulators of G-protein signalling ) are encoded by the SST2 gene of the yeast Saccharomyces cerevisiae , the EGL-10 gene of the nematode Caenorhabdatis elegans , and several related mammalian genes .
	manualset3
126293	7	405283	5	NULL	NULL	0	NULL	nematode Caenorhabdatis elegans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Polypeptides that define a protein family termed RGS ( for regulators of G-protein signalling ) are encoded by the SST2 gene of the yeast Saccharomyces cerevisiae , the EGL-10 gene of the nematode Caenorhabdatis elegans , and several related mammalian genes .
	manualset3
126294	8	405283	5	NULL	NULL	0	NULL	mammalian genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Polypeptides that define a protein family termed RGS ( for regulators of G-protein signalling ) are encoded by the SST2 gene of the yeast Saccharomyces cerevisiae , the EGL-10 gene of the nematode Caenorhabdatis elegans , and several related mammalian genes .
	manualset3
126295	1	405284	5	NULL	NULL	0	NULL	Polyphenolic composition	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyphenolic composition of two Syrah wines aged during 6 or 12 months in medium toasting acacia and oak 225L barrels was studied by LC-DAD-ESI/MS .
	manualset3
126296	2	405284	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyphenolic composition of two Syrah wines aged during 6 or 12 months in medium toasting acacia and oak 225L barrels was studied by LC-DAD-ESI/MS .
	manualset3
126297	3	405284	5	NULL	NULL	0	NULL	Syrah wines	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyphenolic composition of two Syrah wines aged during 6 or 12 months in medium toasting acacia and oak 225L barrels was studied by LC-DAD-ESI/MS .
	manualset3
126298	4	405284	5	NULL	NULL	0	NULL	6 or 12 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyphenolic composition of two Syrah wines aged during 6 or 12 months in medium toasting acacia and oak 225L barrels was studied by LC-DAD-ESI/MS .
	manualset3
126299	5	405284	5	NULL	NULL	NULL	NULL	acacia 225L barrels	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Polyphenolic composition of two Syrah wines aged during 6 or 12 months in medium toasting acacia and oak 225L barrels was studied by LC-DAD-ESI/MS .
	manualset3
126300	6	405284	5	NULL	NULL	0	NULL	oak 225L barrels	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyphenolic composition of two Syrah wines aged during 6 or 12 months in medium toasting acacia and oak 225L barrels was studied by LC-DAD-ESI/MS .
	manualset3
126301	7	405284	5	NULL	NULL	0	NULL	LC-DAD-ESI/MS	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyphenolic composition of two Syrah wines aged during 6 or 12 months in medium toasting acacia and oak 225L barrels was studied by LC-DAD-ESI/MS .
	manualset3
126302	1	405285	5	NULL	NULL	0	NULL	Polyribosomes 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyribosomes dissociated from the surface of the membrane by detergent treatment were placed into an amino-acid incorporating system .
	manualset3
126303	2	405285	5	NULL	NULL	0	NULL	surface of the membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyribosomes dissociated from the surface of the membrane by detergent treatment were placed into an amino-acid incorporating system .
	manualset3
126304	3	405285	5	NULL	NULL	0	NULL	detergent treatment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyribosomes dissociated from the surface of the membrane by detergent treatment were placed into an amino-acid incorporating system .
	manualset3
126305	4	405285	5	NULL	NULL	0	NULL	amino-acid incorporating system	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyribosomes dissociated from the surface of the membrane by detergent treatment were placed into an amino-acid incorporating system .
	manualset3
126306	1	405286	5	NULL	NULL	0	NULL	Polysulfide reduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Polysulfide reduction is catalyzed by the membrane-bound polysulfide reductase complex encoded by the psrABC operon .
	manualset3
126307	2	405286	5	NULL	NULL	0	NULL	membrane-bound polysulfide reductase complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Polysulfide reduction is catalyzed by the membrane-bound polysulfide reductase complex encoded by the psrABC operon .
	manualset3
126308	3	405286	5	NULL	NULL	0	NULL	 psrABC operon	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Polysulfide reduction is catalyzed by the membrane-bound polysulfide reductase complex encoded by the psrABC operon .
	manualset3
126309	1	405287	5	NULL	NULL	0	NULL	Polyuridylic acid	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyuridylic acid was effective as messenger RNA with all three ribosomes but much greater stimulation was obtained with ribosomes from E. coli and the hepatoma .
	manualset3
126310	2	405287	5	NULL	NULL	0	NULL	messenger RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyuridylic acid was effective as messenger RNA with all three ribosomes but much greater stimulation was obtained with ribosomes from E. coli and the hepatoma .
	manualset3
126311	3	405287	5	NULL	NULL	0	NULL	three 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyuridylic acid was effective as messenger RNA with all three ribosomes but much greater stimulation was obtained with ribosomes from E. coli and the hepatoma .
	manualset3
126312	4	405287	5	NULL	NULL	0	NULL	ribosomes 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyuridylic acid was effective as messenger RNA with all three ribosomes but much greater stimulation was obtained with ribosomes from E. coli and the hepatoma .
	manualset3
126313	5	405287	5	NULL	NULL	0	NULL	stimulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyuridylic acid was effective as messenger RNA with all three ribosomes but much greater stimulation was obtained with ribosomes from E. coli and the hepatoma .
	manualset3
126314	6	405287	5	NULL	NULL	0	NULL	ribosomes 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyuridylic acid was effective as messenger RNA with all three ribosomes but much greater stimulation was obtained with ribosomes from E. coli and the hepatoma .
	manualset3
126315	7	405287	5	NULL	NULL	0	NULL	 E. coli 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyuridylic acid was effective as messenger RNA with all three ribosomes but much greater stimulation was obtained with ribosomes from E. coli and the hepatoma .
	manualset3
126316	8	405287	5	NULL	NULL	0	NULL	hepatoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Polyuridylic acid was effective as messenger RNA with all three ribosomes but much greater stimulation was obtained with ribosomes from E. coli and the hepatoma .
	manualset3
126317	1	405288	5	NULL	NULL	0	NULL	Ponalrestat 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Ponalrestat significantly increased bacterial killing in the diabetic subjects ( Kmax of ponalrestat 75.1 + / - 16.5 vs. placebo 58.2 + / - 20.8 , P = 0.003 ) so that there was no longer any significant difference in Kmax between the control subjects and the diabetic subjects on active treatment .
	manualset3
126318	2	405288	5	NULL	NULL	0	NULL	bacterial killing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ponalrestat significantly increased bacterial killing in the diabetic subjects ( Kmax of ponalrestat 75.1 + / - 16.5 vs. placebo 58.2 + / - 20.8 , P = 0.003 ) so that there was no longer any significant difference in Kmax between the control subjects and the diabetic subjects on active treatment .
	manualset3
126319	3	405288	5	NULL	NULL	0	NULL	diabetic subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ponalrestat significantly increased bacterial killing in the diabetic subjects ( Kmax of ponalrestat 75.1 + / - 16.5 vs. placebo 58.2 + / - 20.8 , P = 0.003 ) so that there was no longer any significant difference in Kmax between the control subjects and the diabetic subjects on active treatment .
	manualset3
126320	4	405288	5	NULL	NULL	0	NULL	Kmax	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ponalrestat significantly increased bacterial killing in the diabetic subjects ( Kmax of ponalrestat 75.1 + / - 16.5 vs. placebo 58.2 + / - 20.8 , P = 0.003 ) so that there was no longer any significant difference in Kmax between the control subjects and the diabetic subjects on active treatment .
	manualset3
126321	5	405288	5	NULL	NULL	0	NULL	ponalrestat 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Ponalrestat significantly increased bacterial killing in the diabetic subjects ( Kmax of ponalrestat 75.1 + / - 16.5 vs. placebo 58.2 + / - 20.8 , P = 0.003 ) so that there was no longer any significant difference in Kmax between the control subjects and the diabetic subjects on active treatment .
	manualset3
126322	6	405288	5	NULL	NULL	0	NULL	75.1 + / - 16.5	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ponalrestat significantly increased bacterial killing in the diabetic subjects ( Kmax of ponalrestat 75.1 + / - 16.5 vs. placebo 58.2 + / - 20.8 , P = 0.003 ) so that there was no longer any significant difference in Kmax between the control subjects and the diabetic subjects on active treatment .
	manualset3
126323	7	405288	5	NULL	NULL	0	NULL	placebo 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ponalrestat significantly increased bacterial killing in the diabetic subjects ( Kmax of ponalrestat 75.1 + / - 16.5 vs. placebo 58.2 + / - 20.8 , P = 0.003 ) so that there was no longer any significant difference in Kmax between the control subjects and the diabetic subjects on active treatment .
	manualset3
126324	8	405288	5	NULL	NULL	0	NULL	 58.2 + / - 20.8 , P = 0.003 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ponalrestat significantly increased bacterial killing in the diabetic subjects ( Kmax of ponalrestat 75.1 + / - 16.5 vs. placebo 58.2 + / - 20.8 , P = 0.003 ) so that there was no longer any significant difference in Kmax between the control subjects and the diabetic subjects on active treatment .
	manualset3
126325	9	405288	5	NULL	NULL	0	NULL	 significant difference 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ponalrestat significantly increased bacterial killing in the diabetic subjects ( Kmax of ponalrestat 75.1 + / - 16.5 vs. placebo 58.2 + / - 20.8 , P = 0.003 ) so that there was no longer any significant difference in Kmax between the control subjects and the diabetic subjects on active treatment .
	manualset3
126326	10	405288	5	NULL	NULL	0	NULL	Kmax 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ponalrestat significantly increased bacterial killing in the diabetic subjects ( Kmax of ponalrestat 75.1 + / - 16.5 vs. placebo 58.2 + / - 20.8 , P = 0.003 ) so that there was no longer any significant difference in Kmax between the control subjects and the diabetic subjects on active treatment .
	manualset3
126327	11	405288	5	NULL	NULL	0	NULL	control subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ponalrestat significantly increased bacterial killing in the diabetic subjects ( Kmax of ponalrestat 75.1 + / - 16.5 vs. placebo 58.2 + / - 20.8 , P = 0.003 ) so that there was no longer any significant difference in Kmax between the control subjects and the diabetic subjects on active treatment .
	manualset3
126328	12	405288	5	NULL	NULL	0	NULL	diabetic subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ponalrestat significantly increased bacterial killing in the diabetic subjects ( Kmax of ponalrestat 75.1 + / - 16.5 vs. placebo 58.2 + / - 20.8 , P = 0.003 ) so that there was no longer any significant difference in Kmax between the control subjects and the diabetic subjects on active treatment .
	manualset3
126329	13	405288	5	NULL	NULL	0	NULL	active treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ponalrestat significantly increased bacterial killing in the diabetic subjects ( Kmax of ponalrestat 75.1 + / - 16.5 vs. placebo 58.2 + / - 20.8 , P = 0.003 ) so that there was no longer any significant difference in Kmax between the control subjects and the diabetic subjects on active treatment .
	manualset3
126330	1	405289	5	NULL	NULL	0	NULL	Pooled conjugated and unconjugated bile acids 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Pooled conjugated and unconjugated bile acids decreased normal lymphocyte E rosette formation in vitro .
	manualset3
126331	2	405289	5	NULL	NULL	0	NULL	normal lymphocyte E rosette formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pooled conjugated and unconjugated bile acids decreased normal lymphocyte E rosette formation in vitro .
	manualset3
126332	1	405290	5	NULL	NULL	0	NULL	individual data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Pooling all the individual data , individual ME values were correlated ( r2 = 0.33 ) with individual food : gain ratios , which shows that a great part of ME variation was associated with individual variation .
	manualset3
126333	2	405290	5	NULL	NULL	0	NULL	individual ME values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pooling all the individual data , individual ME values were correlated ( r2 = 0.33 ) with individual food : gain ratios , which shows that a great part of ME variation was associated with individual variation .
	manualset3
126334	3	405290	5	NULL	NULL	0	NULL	r2 = 0.33	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pooling all the individual data , individual ME values were correlated ( r2 = 0.33 ) with individual food : gain ratios , which shows that a great part of ME variation was associated with individual variation .
	manualset3
126335	4	405290	5	NULL	NULL	0	NULL	individual food : gain ratios	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pooling all the individual data , individual ME values were correlated ( r2 = 0.33 ) with individual food : gain ratios , which shows that a great part of ME variation was associated with individual variation .
	manualset3
126336	5	405290	5	NULL	NULL	0	NULL	ME variation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pooling all the individual data , individual ME values were correlated ( r2 = 0.33 ) with individual food : gain ratios , which shows that a great part of ME variation was associated with individual variation .
	manualset3
126337	6	405290	5	NULL	NULL	0	NULL	individual variation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pooling all the individual data , individual ME values were correlated ( r2 = 0.33 ) with individual food : gain ratios , which shows that a great part of ME variation was associated with individual variation .
	manualset3
126338	1	405291	5	NULL	NULL	0	NULL	Poor venous access	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Poor venous access is even more problematic in very young children , the vast majority of whom will require the insertion of central venous access devices ( CVADs ) .
	manualset3
126339	2	405291	5	NULL	NULL	0	NULL	very young children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Poor venous access is even more problematic in very young children , the vast majority of whom will require the insertion of central venous access devices ( CVADs ) .
	manualset3
126340	3	405291	5	NULL	NULL	0	NULL	majority 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Poor venous access is even more problematic in very young children , the vast majority of whom will require the insertion of central venous access devices ( CVADs ) .
	manualset3
126341	4	405291	5	NULL	NULL	0	NULL	insertion 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Poor venous access is even more problematic in very young children , the vast majority of whom will require the insertion of central venous access devices ( CVADs ) .
	manualset3
126342	5	405291	5	NULL	NULL	0	NULL	central venous access devices ( CVADs )	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Poor venous access is even more problematic in very young children , the vast majority of whom will require the insertion of central venous access devices ( CVADs ) .
	manualset3
126343	1	405292	5	NULL	NULL	0	NULL	Poor laboratory practice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Poor laboratory practice yields compliance issues , increased cost , increased cycle time and delayed product introductions .
	manualset3
126344	2	405292	5	NULL	NULL	0	NULL	compliance issues	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Poor laboratory practice yields compliance issues , increased cost , increased cycle time and delayed product introductions .
	manualset3
126345	3	405292	5	NULL	NULL	NULL	NULL	increased cost	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Poor laboratory practice yields compliance issues , increased cost , increased cycle time and delayed product introductions .
	manualset3
126346	4	405292	5	NULL	NULL	0	NULL	increased cycle time 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Poor laboratory practice yields compliance issues , increased cost , increased cycle time and delayed product introductions .
	manualset3
126347	5	405292	5	NULL	NULL	0	NULL	delayed product introductions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Poor laboratory practice yields compliance issues , increased cost , increased cycle time and delayed product introductions .
	manualset3
126348	1	405293	5	NULL	NULL	0	NULL	Poor TI	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Poor TI could be due to ( 1 ) posttransplant cell loss , ( 2 ) a rare sub-population of cancer stem cells or ( 3 ) a requirement for specific cellular interactions , which rely on cell number .
	manualset3
126349	2	405293	5	NULL	NULL	0	NULL	posttransplant cell loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Poor TI could be due to ( 1 ) posttransplant cell loss , ( 2 ) a rare sub-population of cancer stem cells or ( 3 ) a requirement for specific cellular interactions , which rely on cell number .
	manualset3
126350	3	405293	5	NULL	NULL	0	NULL	rare sub-population	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Poor TI could be due to ( 1 ) posttransplant cell loss , ( 2 ) a rare sub-population of cancer stem cells or ( 3 ) a requirement for specific cellular interactions , which rely on cell number .
	manualset3
126351	4	405293	5	NULL	NULL	0	NULL	cancer stem cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Poor TI could be due to ( 1 ) posttransplant cell loss , ( 2 ) a rare sub-population of cancer stem cells or ( 3 ) a requirement for specific cellular interactions , which rely on cell number .
	manualset3
126352	5	405293	5	NULL	NULL	0	NULL	requirement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Poor TI could be due to ( 1 ) posttransplant cell loss , ( 2 ) a rare sub-population of cancer stem cells or ( 3 ) a requirement for specific cellular interactions , which rely on cell number .
	manualset3
126353	6	405293	5	NULL	NULL	0	NULL	specific cellular interactions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Poor TI could be due to ( 1 ) posttransplant cell loss , ( 2 ) a rare sub-population of cancer stem cells or ( 3 ) a requirement for specific cellular interactions , which rely on cell number .
	manualset3
126354	7	405293	5	NULL	NULL	0	NULL	cell number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Poor TI could be due to ( 1 ) posttransplant cell loss , ( 2 ) a rare sub-population of cancer stem cells or ( 3 ) a requirement for specific cellular interactions , which rely on cell number .
	manualset3
126355	1	405294	5	NULL	NULL	0	NULL	recovery	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Poorest recovery of S-13 was obtained at 50 % RH .
	manualset3
126356	2	405294	5	NULL	NULL	0	NULL	S-13	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Poorest recovery of S-13 was obtained at 50 % RH .
	manualset3
126357	3	405294	5	NULL	NULL	0	NULL	50 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Poorest recovery of S-13 was obtained at 50 % RH .
	manualset3
126358	4	405294	5	NULL	NULL	0	NULL	RH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Poorest recovery of S-13 was obtained at 50 % RH .
	manualset3
126359	1	405295	5	NULL	NULL	0	NULL	Popliteal artery aneurysms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Popliteal artery aneurysms are the most common peripheral aneurysm .
	manualset3
126360	2	405295	5	NULL	NULL	0	NULL	peripheral aneurysm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Popliteal artery aneurysms are the most common peripheral aneurysm .
	manualset3
126361	1	405296	5	NULL	NULL	0	NULL	Population pharmacokinetics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Population pharmacokinetics of amikacin in critically ill patients .
	manualset3
126362	2	405296	5	NULL	NULL	0	NULL	amikacin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Population pharmacokinetics of amikacin in critically ill patients .
	manualset3
126363	3	405296	5	NULL	NULL	0	NULL	critically ill patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Population pharmacokinetics of amikacin in critically ill patients .
	manualset3
126364	1	405297	5	NULL	NULL	0	NULL	human high-density complementary DNA ( cDNA ) microarray	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A human high-density complementary DNA ( cDNA ) microarray consisting of 9 , 182 probes was used to compare gene transcription profiles of LM between the two breeds .
	manualset3
126365	2	405297	5	NULL	NULL	0	NULL	9 , 182 probes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A human high-density complementary DNA ( cDNA ) microarray consisting of 9 , 182 probes was used to compare gene transcription profiles of LM between the two breeds .
	manualset3
126366	3	405297	5	NULL	NULL	0	NULL	gene transcription profiles	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A human high-density complementary DNA ( cDNA ) microarray consisting of 9 , 182 probes was used to compare gene transcription profiles of LM between the two breeds .
	manualset3
126367	4	405297	5	NULL	NULL	NULL	NULL	LM 	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A human high-density complementary DNA ( cDNA ) microarray consisting of 9 , 182 probes was used to compare gene transcription profiles of LM between the two breeds .
	manualset3
126368	5	405297	5	NULL	NULL	0	NULL	two breeds	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A human high-density complementary DNA ( cDNA ) microarray consisting of 9 , 182 probes was used to compare gene transcription profiles of LM between the two breeds .
	manualset3
126369	1	405298	5	NULL	NULL	0	NULL	Population study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Population study of dihydropyrimidine dehydrogenase in cancer patients .
	manualset3
126370	2	405298	5	NULL	NULL	0	NULL	dihydropyrimidine dehydrogenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Population study of dihydropyrimidine dehydrogenase in cancer patients .
	manualset3
126371	3	405298	5	NULL	NULL	0	NULL	cancer patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Population study of dihydropyrimidine dehydrogenase in cancer patients .
	manualset3
126372	1	405299	5	NULL	NULL	0	NULL	Pore size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pore size and negative charge as structural determinants of permeability in the Torpedo nicotinic acetylcholine receptor channel .
	manualset3
126373	2	405299	5	NULL	NULL	0	NULL	negative charge	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pore size and negative charge as structural determinants of permeability in the Torpedo nicotinic acetylcholine receptor channel .
	manualset3
126374	3	405299	5	NULL	NULL	0	NULL	structural determinants	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pore size and negative charge as structural determinants of permeability in the Torpedo nicotinic acetylcholine receptor channel .
	manualset3
126375	4	405299	5	NULL	NULL	0	NULL	permeability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pore size and negative charge as structural determinants of permeability in the Torpedo nicotinic acetylcholine receptor channel .
	manualset3
126376	5	405299	5	NULL	NULL	0	NULL	Torpedo nicotinic acetylcholine receptor channel	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Pore size and negative charge as structural determinants of permeability in the Torpedo nicotinic acetylcholine receptor channel .
	manualset3
126377	1	405300	5	NULL	NULL	0	NULL	Porphyria cutanea tarda	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Porphyria cutanea tarda is the most frequent porphyria and occurs in both sporadic and familial forms .
	manualset3
126378	2	405300	5	NULL	NULL	0	NULL	porphyria	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Porphyria cutanea tarda is the most frequent porphyria and occurs in both sporadic and familial forms .
	manualset3
126379	3	405300	5	NULL	NULL	0	NULL	sporadic form	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Porphyria cutanea tarda is the most frequent porphyria and occurs in both sporadic and familial forms .
	manualset3
126380	4	405300	5	NULL	NULL	0	NULL	familial form	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Porphyria cutanea tarda is the most frequent porphyria and occurs in both sporadic and familial forms .
	manualset3
126381	1	405301	5	NULL	NULL	0	NULL	Portal-systemic shunt	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Portal-systemic shunt in hepatic cirrhosis : does the type of shunt decisively influence the clinical result ?
	manualset3
126382	2	405301	5	NULL	NULL	0	NULL	hepatic cirrhosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Portal-systemic shunt in hepatic cirrhosis : does the type of shunt decisively influence the clinical result ?
	manualset3
126383	3	405301	5	NULL	NULL	0	NULL	type	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Portal-systemic shunt in hepatic cirrhosis : does the type of shunt decisively influence the clinical result ?
	manualset3
126384	4	405301	5	NULL	NULL	0	NULL	shunt	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Portal-systemic shunt in hepatic cirrhosis : does the type of shunt decisively influence the clinical result ?
	manualset3
126386	6	405301	5	NULL	NULL	0	NULL	clinical result	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Portal-systemic shunt in hepatic cirrhosis : does the type of shunt decisively influence the clinical result ?
	manualset3
126387	1	405302	5	NULL	NULL	0	NULL	Portions	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Portions of an adult human lung were studied by autoradiography in order to detect the presence of fallout particles .
	manualset3
126388	2	405302	5	NULL	NULL	0	NULL	 adult human lung 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Portions of an adult human lung were studied by autoradiography in order to detect the presence of fallout particles .
	manualset3
126389	3	405302	5	NULL	NULL	0	NULL	autoradiography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Portions of an adult human lung were studied by autoradiography in order to detect the presence of fallout particles .
	manualset3
126390	4	405302	5	NULL	NULL	0	NULL	order	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Portions of an adult human lung were studied by autoradiography in order to detect the presence of fallout particles .
	manualset3
126391	5	405302	5	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Portions of an adult human lung were studied by autoradiography in order to detect the presence of fallout particles .
	manualset3
126392	6	405302	5	NULL	NULL	0	NULL	fallout particles	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Portions of an adult human lung were studied by autoradiography in order to detect the presence of fallout particles .
	manualset3
126508	1	405303	5	NULL	NULL	0	NULL	Portopulmonary hypertension syndrome ( PPHS )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Portopulmonary hypertension syndrome ( PPHS ) is a complication of portal hypertension where the substrate is micro-vessel lesions which are indicative of plexogenic arteriopathy .
	manualset3
126509	2	405303	5	NULL	NULL	0	NULL	complication 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Portopulmonary hypertension syndrome ( PPHS ) is a complication of portal hypertension where the substrate is micro-vessel lesions which are indicative of plexogenic arteriopathy .
	manualset3
126510	3	405303	5	NULL	NULL	0	NULL	portal hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Portopulmonary hypertension syndrome ( PPHS ) is a complication of portal hypertension where the substrate is micro-vessel lesions which are indicative of plexogenic arteriopathy .
	manualset3
126511	4	405303	5	NULL	NULL	0	NULL	substrate 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Portopulmonary hypertension syndrome ( PPHS ) is a complication of portal hypertension where the substrate is micro-vessel lesions which are indicative of plexogenic arteriopathy .
	manualset3
126512	5	405303	5	NULL	NULL	0	NULL	micro-vessel lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Portopulmonary hypertension syndrome ( PPHS ) is a complication of portal hypertension where the substrate is micro-vessel lesions which are indicative of plexogenic arteriopathy .
	manualset3
126513	6	405303	5	NULL	NULL	0	NULL	plexogenic arteriopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Portopulmonary hypertension syndrome ( PPHS ) is a complication of portal hypertension where the substrate is micro-vessel lesions which are indicative of plexogenic arteriopathy .
	manualset3
126393	1	405304	5	NULL	NULL	0	NULL	Positive IgM antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive IgM antibodies to the viral capsule antigen followed by marked elevation of the IgG fraction suggest chronic Epstein-Barr virus infection to be the etiology .
	manualset3
126394	2	405304	5	NULL	NULL	0	NULL	viral capsule antigen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive IgM antibodies to the viral capsule antigen followed by marked elevation of the IgG fraction suggest chronic Epstein-Barr virus infection to be the etiology .
	manualset3
126395	3	405304	5	NULL	NULL	0	NULL	elevation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive IgM antibodies to the viral capsule antigen followed by marked elevation of the IgG fraction suggest chronic Epstein-Barr virus infection to be the etiology .
	manualset3
126396	4	405304	5	NULL	NULL	0	NULL	IgG fraction	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive IgM antibodies to the viral capsule antigen followed by marked elevation of the IgG fraction suggest chronic Epstein-Barr virus infection to be the etiology .
	manualset3
126397	5	405304	5	NULL	NULL	0	NULL	chronic Epstein-Barr virus infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive IgM antibodies to the viral capsule antigen followed by marked elevation of the IgG fraction suggest chronic Epstein-Barr virus infection to be the etiology .
	manualset3
126398	6	405304	5	NULL	NULL	0	NULL	etiology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive IgM antibodies to the viral capsule antigen followed by marked elevation of the IgG fraction suggest chronic Epstein-Barr virus infection to be the etiology .
	manualset3
126399	1	405305	5	NULL	NULL	0	NULL	Positive PCNA immunostaining	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive PCNA immunostaining , along with the presence of mitotic figures , indicated that EVT cells in vitro retained the ability for cell proliferation .
	manualset3
126400	2	405305	5	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive PCNA immunostaining , along with the presence of mitotic figures , indicated that EVT cells in vitro retained the ability for cell proliferation .
	manualset3
126401	3	405305	5	NULL	NULL	0	NULL	mitotic figures 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive PCNA immunostaining , along with the presence of mitotic figures , indicated that EVT cells in vitro retained the ability for cell proliferation .
	manualset3
126402	4	405305	5	NULL	NULL	0	NULL	EVT cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive PCNA immunostaining , along with the presence of mitotic figures , indicated that EVT cells in vitro retained the ability for cell proliferation .
	manualset3
126403	5	405305	5	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive PCNA immunostaining , along with the presence of mitotic figures , indicated that EVT cells in vitro retained the ability for cell proliferation .
	manualset3
126404	6	405305	5	NULL	NULL	0	NULL	cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive PCNA immunostaining , along with the presence of mitotic figures , indicated that EVT cells in vitro retained the ability for cell proliferation .
	manualset3
126405	1	405306	5	NULL	NULL	0	NULL	Positive alleles	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive alleles for GPC at these loci were contributed by the high-GPC parent Strongfield .
	manualset3
126406	2	405306	5	NULL	NULL	0	NULL	GPC	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive alleles for GPC at these loci were contributed by the high-GPC parent Strongfield .
	manualset3
126407	3	405306	5	NULL	NULL	0	NULL	loci	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive alleles for GPC at these loci were contributed by the high-GPC parent Strongfield .
	manualset3
126408	4	405306	5	NULL	NULL	0	NULL	high-GPC parent Strongfield	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive alleles for GPC at these loci were contributed by the high-GPC parent Strongfield .
	manualset3
126409	1	405307	5	NULL	NULL	0	NULL	Positive associations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive associations of the 5-HTTLPR polymorphism with autism have been reported by two family-based studies , but one found preferential transmission of the short allele and the other of the long allele .
	manualset3
126410	2	405307	5	NULL	NULL	0	NULL	5-HTTLPR polymorphism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive associations of the 5-HTTLPR polymorphism with autism have been reported by two family-based studies , but one found preferential transmission of the short allele and the other of the long allele .
	manualset3
126411	3	405307	5	NULL	NULL	0	NULL	autism	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive associations of the 5-HTTLPR polymorphism with autism have been reported by two family-based studies , but one found preferential transmission of the short allele and the other of the long allele .
	manualset3
126412	4	405307	5	NULL	NULL	0	NULL	two	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive associations of the 5-HTTLPR polymorphism with autism have been reported by two family-based studies , but one found preferential transmission of the short allele and the other of the long allele .
	manualset3
126413	5	405307	5	NULL	NULL	0	NULL	family-based studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive associations of the 5-HTTLPR polymorphism with autism have been reported by two family-based studies , but one found preferential transmission of the short allele and the other of the long allele .
	manualset3
126414	6	405307	5	NULL	NULL	0	NULL	preferential transmission	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive associations of the 5-HTTLPR polymorphism with autism have been reported by two family-based studies , but one found preferential transmission of the short allele and the other of the long allele .
	manualset3
126415	7	405307	5	NULL	NULL	0	NULL	short allele	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive associations of the 5-HTTLPR polymorphism with autism have been reported by two family-based studies , but one found preferential transmission of the short allele and the other of the long allele .
	manualset3
126416	8	405307	5	NULL	NULL	0	NULL	long allele	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive associations of the 5-HTTLPR polymorphism with autism have been reported by two family-based studies , but one found preferential transmission of the short allele and the other of the long allele .
	manualset3
126417	1	405308	5	NULL	NULL	0	NULL	Positive cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive cells , identified with a panel of antisera raised against four different regions of the prosomatostatin molecule , were found in 100 % of the tumors .
	manualset3
126418	2	405308	5	NULL	NULL	0	NULL	panel	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive cells , identified with a panel of antisera raised against four different regions of the prosomatostatin molecule , were found in 100 % of the tumors .
	manualset3
126419	3	405308	5	NULL	NULL	0	NULL	antisera	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive cells , identified with a panel of antisera raised against four different regions of the prosomatostatin molecule , were found in 100 % of the tumors .
	manualset3
126420	4	405308	5	NULL	NULL	0	NULL	four	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive cells , identified with a panel of antisera raised against four different regions of the prosomatostatin molecule , were found in 100 % of the tumors .
	manualset3
126421	5	405308	5	NULL	NULL	0	NULL	different regions	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive cells , identified with a panel of antisera raised against four different regions of the prosomatostatin molecule , were found in 100 % of the tumors .
	manualset3
126422	6	405308	5	NULL	NULL	0	NULL	prosomatostatin molecule	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive cells , identified with a panel of antisera raised against four different regions of the prosomatostatin molecule , were found in 100 % of the tumors .
	manualset3
126423	7	405308	5	NULL	NULL	0	NULL	100 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive cells , identified with a panel of antisera raised against four different regions of the prosomatostatin molecule , were found in 100 % of the tumors .
	manualset3
126424	8	405308	5	NULL	NULL	0	NULL	tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive cells , identified with a panel of antisera raised against four different regions of the prosomatostatin molecule , were found in 100 % of the tumors .
	manualset3
126425	1	405309	5	NULL	NULL	0	NULL	Positive fecal specimens	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive fecal specimens and nonautoclaved rodent diet both contained a substance that apparently attached nonspecifically to the antibody coated beads used in the ELISA and reacted directly with the substrate in the absence of the conjugate .
	manualset3
126426	2	405309	5	NULL	NULL	0	NULL	nonautoclaved rodent diet 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive fecal specimens and nonautoclaved rodent diet both contained a substance that apparently attached nonspecifically to the antibody coated beads used in the ELISA and reacted directly with the substrate in the absence of the conjugate .
	manualset3
126427	3	405309	5	NULL	NULL	NULL	NULL	substance	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Positive fecal specimens and nonautoclaved rodent diet both contained a substance that apparently attached nonspecifically to the antibody coated beads used in the ELISA and reacted directly with the substrate in the absence of the conjugate .
	manualset3
126428	4	405309	5	NULL	NULL	0	NULL	antibody coated beads	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive fecal specimens and nonautoclaved rodent diet both contained a substance that apparently attached nonspecifically to the antibody coated beads used in the ELISA and reacted directly with the substrate in the absence of the conjugate .
	manualset3
126429	5	405309	5	NULL	NULL	0	NULL	ELISA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive fecal specimens and nonautoclaved rodent diet both contained a substance that apparently attached nonspecifically to the antibody coated beads used in the ELISA and reacted directly with the substrate in the absence of the conjugate .
	manualset3
126430	6	405309	5	NULL	NULL	NULL	NULL	substrate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Positive fecal specimens and nonautoclaved rodent diet both contained a substance that apparently attached nonspecifically to the antibody coated beads used in the ELISA and reacted directly with the substrate in the absence of the conjugate .
	manualset3
126431	7	405309	5	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive fecal specimens and nonautoclaved rodent diet both contained a substance that apparently attached nonspecifically to the antibody coated beads used in the ELISA and reacted directly with the substrate in the absence of the conjugate .
	manualset3
126432	8	405309	5	NULL	NULL	0	NULL	conjugate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive fecal specimens and nonautoclaved rodent diet both contained a substance that apparently attached nonspecifically to the antibody coated beads used in the ELISA and reacted directly with the substrate in the absence of the conjugate .
	manualset3
126433	1	405310	5	NULL	NULL	0	NULL	Positive findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive findings on SMRCP were observed in all MPBM patients .
	manualset3
126434	2	405310	5	NULL	NULL	0	NULL	SMRCP	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive findings on SMRCP were observed in all MPBM patients .
	manualset3
126435	3	405310	5	NULL	NULL	0	NULL	MPBM patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive findings on SMRCP were observed in all MPBM patients .
	manualset3
126436	1	405311	5	NULL	NULL	0	NULL	Positive health-related changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive health-related changes included an increase in fruit and vegetable intake , food preparation using less grease , and baking rather than frying .
	manualset3
126437	2	405311	5	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive health-related changes included an increase in fruit and vegetable intake , food preparation using less grease , and baking rather than frying .
	manualset3
126438	3	405311	5	NULL	NULL	0	NULL	fruit and vegetable intake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive health-related changes included an increase in fruit and vegetable intake , food preparation using less grease , and baking rather than frying .
	manualset3
126439	4	405311	5	NULL	NULL	0	NULL	food preparation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive health-related changes included an increase in fruit and vegetable intake , food preparation using less grease , and baking rather than frying .
	manualset3
126440	5	405311	5	NULL	NULL	0	NULL	grease 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive health-related changes included an increase in fruit and vegetable intake , food preparation using less grease , and baking rather than frying .
	manualset3
126441	6	405311	5	NULL	NULL	0	NULL	baking 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive health-related changes included an increase in fruit and vegetable intake , food preparation using less grease , and baking rather than frying .
	manualset3
126442	7	405311	5	NULL	NULL	0	NULL	frying 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive health-related changes included an increase in fruit and vegetable intake , food preparation using less grease , and baking rather than frying .
	manualset3
126443	1	405312	5	NULL	NULL	0	NULL	Positive selection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive selection is known to dominate intra-host evolution of HIV-1 , whereas high genetic variability underlies the belief that neutral processes drive inter-host differences .
	manualset3
126444	2	405312	5	NULL	NULL	0	NULL	intra-host evolution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive selection is known to dominate intra-host evolution of HIV-1 , whereas high genetic variability underlies the belief that neutral processes drive inter-host differences .
	manualset3
126445	3	405312	5	NULL	NULL	0	NULL	HIV-1	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive selection is known to dominate intra-host evolution of HIV-1 , whereas high genetic variability underlies the belief that neutral processes drive inter-host differences .
	manualset3
126446	4	405312	5	NULL	NULL	0	NULL	high genetic variability	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive selection is known to dominate intra-host evolution of HIV-1 , whereas high genetic variability underlies the belief that neutral processes drive inter-host differences .
	manualset3
126447	5	405312	5	NULL	NULL	0	NULL	belief 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive selection is known to dominate intra-host evolution of HIV-1 , whereas high genetic variability underlies the belief that neutral processes drive inter-host differences .
	manualset3
126448	6	405312	5	NULL	NULL	NULL	NULL	neutral processes	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Positive selection is known to dominate intra-host evolution of HIV-1 , whereas high genetic variability underlies the belief that neutral processes drive inter-host differences .
	manualset3
126449	7	405312	5	NULL	NULL	0	NULL	inter-host differences	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive selection is known to dominate intra-host evolution of HIV-1 , whereas high genetic variability underlies the belief that neutral processes drive inter-host differences .
	manualset3
126450	1	405313	5	NULL	NULL	0	NULL	Positive specific pharmacodynamic interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive specific pharmacodynamic interaction was therefore most marked in isolates with reduced sensitivity against artemisinin and DBB .
	manualset3
126451	2	405313	5	NULL	NULL	NULL	NULL	isolates 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Positive specific pharmacodynamic interaction was therefore most marked in isolates with reduced sensitivity against artemisinin and DBB .
	manualset3
126452	3	405313	5	NULL	NULL	0	NULL	reduced sensitivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive specific pharmacodynamic interaction was therefore most marked in isolates with reduced sensitivity against artemisinin and DBB .
	manualset3
126453	4	405313	5	NULL	NULL	0	NULL	artemisinin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive specific pharmacodynamic interaction was therefore most marked in isolates with reduced sensitivity against artemisinin and DBB .
	manualset3
126454	5	405313	5	NULL	NULL	0	NULL	DBB 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive specific pharmacodynamic interaction was therefore most marked in isolates with reduced sensitivity against artemisinin and DBB .
	manualset3
126455	1	405314	5	NULL	NULL	0	NULL	hydrophobic sequence ( called here the VFV motif )	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A hydrophobic sequence ( called here the VFV motif ) is conserved among GM , the liver subunit GL , and the widely expressed subunits , PTG , R5 and U5 .
	manualset3
126456	2	405314	5	NULL	NULL	NULL	NULL	GM	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A hydrophobic sequence ( called here the VFV motif ) is conserved among GM , the liver subunit GL , and the widely expressed subunits , PTG , R5 and U5 .
	manualset3
126457	3	405314	5	NULL	NULL	0	NULL	 liver subunit GL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A hydrophobic sequence ( called here the VFV motif ) is conserved among GM , the liver subunit GL , and the widely expressed subunits , PTG , R5 and U5 .
	manualset3
126458	4	405314	5	NULL	NULL	0	NULL	widely expressed subunits	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A hydrophobic sequence ( called here the VFV motif ) is conserved among GM , the liver subunit GL , and the widely expressed subunits , PTG , R5 and U5 .
	manualset3
126459	5	405314	5	NULL	NULL	0	NULL	PTG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A hydrophobic sequence ( called here the VFV motif ) is conserved among GM , the liver subunit GL , and the widely expressed subunits , PTG , R5 and U5 .
	manualset3
126460	6	405314	5	NULL	NULL	0	NULL	R5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A hydrophobic sequence ( called here the VFV motif ) is conserved among GM , the liver subunit GL , and the widely expressed subunits , PTG , R5 and U5 .
	manualset3
126461	7	405314	5	NULL	NULL	0	NULL	U5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A hydrophobic sequence ( called here the VFV motif ) is conserved among GM , the liver subunit GL , and the widely expressed subunits , PTG , R5 and U5 .
	manualset3
126462	1	405315	5	NULL	NULL	0	NULL	Positive staining	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive staining with 4H84 mAb was detected in acid-treated cells isolated from 16 out of 30 patients .
	manualset3
126463	2	405315	5	NULL	NULL	0	NULL	4H84 mAb	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive staining with 4H84 mAb was detected in acid-treated cells isolated from 16 out of 30 patients .
	manualset3
126464	3	405315	5	NULL	NULL	0	NULL	acid-treated cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive staining with 4H84 mAb was detected in acid-treated cells isolated from 16 out of 30 patients .
	manualset3
126465	4	405315	5	NULL	NULL	0	NULL	16 out of 30 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive staining with 4H84 mAb was detected in acid-treated cells isolated from 16 out of 30 patients .
	manualset3
126466	5	405315	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Positive staining with 4H84 mAb was detected in acid-treated cells isolated from 16 out of 30 patients .
	manualset3
126467	1	405316	5	NULL	NULL	0	NULL	Positivity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Positivity and sensitivity of CDT are superior to those other usual biological parameters .
	manualset3
126468	2	405316	5	NULL	NULL	0	NULL	sensitivity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Positivity and sensitivity of CDT are superior to those other usual biological parameters .
	manualset3
126469	3	405316	5	NULL	NULL	0	NULL	CDT 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Positivity and sensitivity of CDT are superior to those other usual biological parameters .
	manualset3
126470	4	405316	5	NULL	NULL	0	NULL	biological parameters	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Positivity and sensitivity of CDT are superior to those other usual biological parameters .
	manualset3
126471	1	405317	5	NULL	NULL	0	NULL	Positron emission tomography studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Positron emission tomography studies using the SERT ligand ( ( 11 ) C ) DASB and the 5-HT ( 2A ) receptor ligand ( ( 11 ) C ) MDL 100907 were evaluated in 13 current and recently detoxified MDMA users and 13 matched healthy controls .
	manualset3
126472	2	405317	5	NULL	NULL	0	NULL	SERT ligand ( ( 11 ) C ) DASB	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Positron emission tomography studies using the SERT ligand ( ( 11 ) C ) DASB and the 5-HT ( 2A ) receptor ligand ( ( 11 ) C ) MDL 100907 were evaluated in 13 current and recently detoxified MDMA users and 13 matched healthy controls .
	manualset3
126473	3	405317	5	NULL	NULL	0	NULL	5-HT ( 2A ) receptor ligand ( ( 11 ) C ) MDL 100907	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Positron emission tomography studies using the SERT ligand ( ( 11 ) C ) DASB and the 5-HT ( 2A ) receptor ligand ( ( 11 ) C ) MDL 100907 were evaluated in 13 current and recently detoxified MDMA users and 13 matched healthy controls .
	manualset3
126474	4	405317	5	NULL	NULL	0	NULL	13	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Positron emission tomography studies using the SERT ligand ( ( 11 ) C ) DASB and the 5-HT ( 2A ) receptor ligand ( ( 11 ) C ) MDL 100907 were evaluated in 13 current and recently detoxified MDMA users and 13 matched healthy controls .
	manualset3
126475	5	405317	5	NULL	NULL	0	NULL	current and recently detoxified MDMA users	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Positron emission tomography studies using the SERT ligand ( ( 11 ) C ) DASB and the 5-HT ( 2A ) receptor ligand ( ( 11 ) C ) MDL 100907 were evaluated in 13 current and recently detoxified MDMA users and 13 matched healthy controls .
	manualset3
126476	6	405317	5	NULL	NULL	0	NULL	13	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Positron emission tomography studies using the SERT ligand ( ( 11 ) C ) DASB and the 5-HT ( 2A ) receptor ligand ( ( 11 ) C ) MDL 100907 were evaluated in 13 current and recently detoxified MDMA users and 13 matched healthy controls .
	manualset3
126477	7	405317	5	NULL	NULL	0	NULL	matched healthy controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Positron emission tomography studies using the SERT ligand ( ( 11 ) C ) DASB and the 5-HT ( 2A ) receptor ligand ( ( 11 ) C ) MDL 100907 were evaluated in 13 current and recently detoxified MDMA users and 13 matched healthy controls .
	manualset3
126478	1	405318	5	NULL	NULL	0	NULL	changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible changes in the level of mRNAs encoding the neuropeptides somatostatin ( SOM ) and neuropeptide Y ( NPY ) were also studied .
	manualset3
126479	2	405318	5	NULL	NULL	0	NULL	level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible changes in the level of mRNAs encoding the neuropeptides somatostatin ( SOM ) and neuropeptide Y ( NPY ) were also studied .
	manualset3
126480	3	405318	5	NULL	NULL	0	NULL	mRNAs encoding the neuropeptides somatostatin ( SOM ) 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible changes in the level of mRNAs encoding the neuropeptides somatostatin ( SOM ) and neuropeptide Y ( NPY ) were also studied .
	manualset3
126481	4	405318	5	NULL	NULL	0	NULL	mRNAs encoding neuropeptide Y ( NPY )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible changes in the level of mRNAs encoding the neuropeptides somatostatin ( SOM ) and neuropeptide Y ( NPY ) were also studied .
	manualset3
126482	1	405319	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible effects of Se on absorption , storage and desaturation of fatty acids were also discussed .
	manualset3
126483	2	405319	5	NULL	NULL	0	NULL	Se	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible effects of Se on absorption , storage and desaturation of fatty acids were also discussed .
	manualset3
126484	3	405319	5	NULL	NULL	0	NULL	absorption 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible effects of Se on absorption , storage and desaturation of fatty acids were also discussed .
	manualset3
126485	4	405319	5	NULL	NULL	0	NULL	storage 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible effects of Se on absorption , storage and desaturation of fatty acids were also discussed .
	manualset3
126486	5	405319	5	NULL	NULL	0	NULL	desaturation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible effects of Se on absorption , storage and desaturation of fatty acids were also discussed .
	manualset3
126487	6	405319	5	NULL	NULL	0	NULL	fatty acids	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible effects of Se on absorption , storage and desaturation of fatty acids were also discussed .
	manualset3
126488	1	405320	5	NULL	NULL	0	NULL	Possible mechanisms 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible mechanisms of 15.8-kb DNA replication are discussed .
	manualset3
126489	2	405320	5	NULL	NULL	0	NULL	15.8-kb DNA replication	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible mechanisms of 15.8-kb DNA replication are discussed .
	manualset3
126490	1	405321	5	NULL	NULL	0	NULL	Possible molecular evolutionary processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible molecular evolutionary processes that may have led to the operation of the Lx cycle in some mistletoes are discussed .
	manualset3
126491	2	405321	5	NULL	NULL	0	NULL	operation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible molecular evolutionary processes that may have led to the operation of the Lx cycle in some mistletoes are discussed .
	manualset3
126492	3	405321	5	NULL	NULL	0	NULL	Lx cycle	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible molecular evolutionary processes that may have led to the operation of the Lx cycle in some mistletoes are discussed .
	manualset3
126493	4	405321	5	NULL	NULL	0	NULL	mistletoes 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible molecular evolutionary processes that may have led to the operation of the Lx cycle in some mistletoes are discussed .
	manualset3
126494	1	405322	5	NULL	NULL	0	NULL	hypothesis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A hypothesis has been proposed that claims much of the phenomena of decompression sickness ( DCS ) are mediated by the complement system of blood plasma .
	manualset3
126495	2	405322	5	NULL	NULL	0	NULL	phenomena 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A hypothesis has been proposed that claims much of the phenomena of decompression sickness ( DCS ) are mediated by the complement system of blood plasma .
	manualset3
126496	3	405322	5	NULL	NULL	0	NULL	decompression sickness ( DCS )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A hypothesis has been proposed that claims much of the phenomena of decompression sickness ( DCS ) are mediated by the complement system of blood plasma .
	manualset3
126497	4	405322	5	NULL	NULL	0	NULL	complement system 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A hypothesis has been proposed that claims much of the phenomena of decompression sickness ( DCS ) are mediated by the complement system of blood plasma .
	manualset3
126498	5	405322	5	NULL	NULL	0	NULL	blood plasma	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A hypothesis has been proposed that claims much of the phenomena of decompression sickness ( DCS ) are mediated by the complement system of blood plasma .
	manualset3
126514	1	405323	5	NULL	NULL	0	NULL	 preventive and control interventions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible preventive and control interventions include special education programs to increase workers ' use of personal protective equipment such as gloves , increased surveillance for influenza viruses among workers and their animals , recommendations that workers seek medical attention should they develop influenza-like illness , and workers ' priority receipt of annual and pandemic influenza vaccines .
	manualset3
126515	2	405323	5	NULL	NULL	0	NULL	special education programs	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible preventive and control interventions include special education programs to increase workers ' use of personal protective equipment such as gloves , increased surveillance for influenza viruses among workers and their animals , recommendations that workers seek medical attention should they develop influenza-like illness , and workers ' priority receipt of annual and pandemic influenza vaccines .
	manualset3
126516	3	405323	5	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible preventive and control interventions include special education programs to increase workers ' use of personal protective equipment such as gloves , increased surveillance for influenza viruses among workers and their animals , recommendations that workers seek medical attention should they develop influenza-like illness , and workers ' priority receipt of annual and pandemic influenza vaccines .
	manualset3
126517	4	405323	5	NULL	NULL	0	NULL	workers ' use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible preventive and control interventions include special education programs to increase workers ' use of personal protective equipment such as gloves , increased surveillance for influenza viruses among workers and their animals , recommendations that workers seek medical attention should they develop influenza-like illness , and workers ' priority receipt of annual and pandemic influenza vaccines .
	manualset3
126518	5	405323	5	NULL	NULL	0	NULL	personal protective equipment	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible preventive and control interventions include special education programs to increase workers ' use of personal protective equipment such as gloves , increased surveillance for influenza viruses among workers and their animals , recommendations that workers seek medical attention should they develop influenza-like illness , and workers ' priority receipt of annual and pandemic influenza vaccines .
	manualset3
126519	6	405323	5	NULL	NULL	0	NULL	gloves 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible preventive and control interventions include special education programs to increase workers ' use of personal protective equipment such as gloves , increased surveillance for influenza viruses among workers and their animals , recommendations that workers seek medical attention should they develop influenza-like illness , and workers ' priority receipt of annual and pandemic influenza vaccines .
	manualset3
126520	7	405323	5	NULL	NULL	0	NULL	increased surveillance 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible preventive and control interventions include special education programs to increase workers ' use of personal protective equipment such as gloves , increased surveillance for influenza viruses among workers and their animals , recommendations that workers seek medical attention should they develop influenza-like illness , and workers ' priority receipt of annual and pandemic influenza vaccines .
	manualset3
126521	8	405323	5	NULL	NULL	0	NULL	influenza viruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible preventive and control interventions include special education programs to increase workers ' use of personal protective equipment such as gloves , increased surveillance for influenza viruses among workers and their animals , recommendations that workers seek medical attention should they develop influenza-like illness , and workers ' priority receipt of annual and pandemic influenza vaccines .
	manualset3
126522	9	405323	5	NULL	NULL	0	NULL	workers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible preventive and control interventions include special education programs to increase workers ' use of personal protective equipment such as gloves , increased surveillance for influenza viruses among workers and their animals , recommendations that workers seek medical attention should they develop influenza-like illness , and workers ' priority receipt of annual and pandemic influenza vaccines .
	manualset3
126523	10	405323	5	NULL	NULL	0	NULL	animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible preventive and control interventions include special education programs to increase workers ' use of personal protective equipment such as gloves , increased surveillance for influenza viruses among workers and their animals , recommendations that workers seek medical attention should they develop influenza-like illness , and workers ' priority receipt of annual and pandemic influenza vaccines .
	manualset3
126524	11	405323	5	NULL	NULL	0	NULL	recommendations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible preventive and control interventions include special education programs to increase workers ' use of personal protective equipment such as gloves , increased surveillance for influenza viruses among workers and their animals , recommendations that workers seek medical attention should they develop influenza-like illness , and workers ' priority receipt of annual and pandemic influenza vaccines .
	manualset3
126525	12	405323	5	NULL	NULL	0	NULL	workers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible preventive and control interventions include special education programs to increase workers ' use of personal protective equipment such as gloves , increased surveillance for influenza viruses among workers and their animals , recommendations that workers seek medical attention should they develop influenza-like illness , and workers ' priority receipt of annual and pandemic influenza vaccines .
	manualset3
126526	13	405323	5	NULL	NULL	0	NULL	medical attention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible preventive and control interventions include special education programs to increase workers ' use of personal protective equipment such as gloves , increased surveillance for influenza viruses among workers and their animals , recommendations that workers seek medical attention should they develop influenza-like illness , and workers ' priority receipt of annual and pandemic influenza vaccines .
	manualset3
126527	14	405323	5	NULL	NULL	0	NULL	influenza-like illness	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible preventive and control interventions include special education programs to increase workers ' use of personal protective equipment such as gloves , increased surveillance for influenza viruses among workers and their animals , recommendations that workers seek medical attention should they develop influenza-like illness , and workers ' priority receipt of annual and pandemic influenza vaccines .
	manualset3
126528	15	405323	5	NULL	NULL	0	NULL	workers ' priority receipt	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible preventive and control interventions include special education programs to increase workers ' use of personal protective equipment such as gloves , increased surveillance for influenza viruses among workers and their animals , recommendations that workers seek medical attention should they develop influenza-like illness , and workers ' priority receipt of annual and pandemic influenza vaccines .
	manualset3
126529	16	405323	5	NULL	NULL	0	NULL	annual and pandemic influenza vaccines	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible preventive and control interventions include special education programs to increase workers ' use of personal protective equipment such as gloves , increased surveillance for influenza viruses among workers and their animals , recommendations that workers seek medical attention should they develop influenza-like illness , and workers ' priority receipt of annual and pandemic influenza vaccines .
	manualset3
126530	1	405324	5	NULL	NULL	0	NULL	reasons 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible reasons for the persistence throughout life of interglobular spaces in the osseous labyrinth of man and some mammals are discussed .
	manualset3
126531	2	405324	5	NULL	NULL	0	NULL	persistence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible reasons for the persistence throughout life of interglobular spaces in the osseous labyrinth of man and some mammals are discussed .
	manualset3
126532	3	405324	5	NULL	NULL	0	NULL	life 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible reasons for the persistence throughout life of interglobular spaces in the osseous labyrinth of man and some mammals are discussed .
	manualset3
126533	4	405324	5	NULL	NULL	0	NULL	interglobular spaces	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible reasons for the persistence throughout life of interglobular spaces in the osseous labyrinth of man and some mammals are discussed .
	manualset3
126534	5	405324	5	NULL	NULL	0	NULL	osseous labyrinth	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible reasons for the persistence throughout life of interglobular spaces in the osseous labyrinth of man and some mammals are discussed .
	manualset3
126535	6	405324	5	NULL	NULL	0	NULL	man 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible reasons for the persistence throughout life of interglobular spaces in the osseous labyrinth of man and some mammals are discussed .
	manualset3
126536	7	405324	5	NULL	NULL	0	NULL	mammals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Possible reasons for the persistence throughout life of interglobular spaces in the osseous labyrinth of man and some mammals are discussed .
	manualset3
126537	1	405325	5	NULL	NULL	0	NULL	Post-OHT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-OHT , case patients received a combination of sildenafil , iloprost , and inhaled nitric oxide .
	manualset3
126538	2	405325	5	NULL	NULL	0	NULL	case patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-OHT , case patients received a combination of sildenafil , iloprost , and inhaled nitric oxide .
	manualset3
126539	3	405325	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-OHT , case patients received a combination of sildenafil , iloprost , and inhaled nitric oxide .
	manualset3
126540	4	405325	5	NULL	NULL	0	NULL	sildenafil 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-OHT , case patients received a combination of sildenafil , iloprost , and inhaled nitric oxide .
	manualset3
126541	5	405325	5	NULL	NULL	0	NULL	iloprost 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-OHT , case patients received a combination of sildenafil , iloprost , and inhaled nitric oxide .
	manualset3
126542	6	405325	5	NULL	NULL	0	NULL	inhaled nitric oxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-OHT , case patients received a combination of sildenafil , iloprost , and inhaled nitric oxide .
	manualset3
126543	1	405326	5	NULL	NULL	0	NULL	Post-flight analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-flight analysis included studies of cell formation , division rate , chemical composition , and ultrastructural organization of cells and their major organelles in weightlessness and hypergravity .
	manualset3
126544	2	405326	5	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-flight analysis included studies of cell formation , division rate , chemical composition , and ultrastructural organization of cells and their major organelles in weightlessness and hypergravity .
	manualset3
126545	3	405326	5	NULL	NULL	0	NULL	cell formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-flight analysis included studies of cell formation , division rate , chemical composition , and ultrastructural organization of cells and their major organelles in weightlessness and hypergravity .
	manualset3
126546	4	405326	5	NULL	NULL	0	NULL	division rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-flight analysis included studies of cell formation , division rate , chemical composition , and ultrastructural organization of cells and their major organelles in weightlessness and hypergravity .
	manualset3
126547	5	405326	5	NULL	NULL	0	NULL	chemical composition	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-flight analysis included studies of cell formation , division rate , chemical composition , and ultrastructural organization of cells and their major organelles in weightlessness and hypergravity .
	manualset3
126548	6	405326	5	NULL	NULL	0	NULL	ultrastructural organization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-flight analysis included studies of cell formation , division rate , chemical composition , and ultrastructural organization of cells and their major organelles in weightlessness and hypergravity .
	manualset3
126549	7	405326	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-flight analysis included studies of cell formation , division rate , chemical composition , and ultrastructural organization of cells and their major organelles in weightlessness and hypergravity .
	manualset3
126550	8	405326	5	NULL	NULL	0	NULL	major organelles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-flight analysis included studies of cell formation , division rate , chemical composition , and ultrastructural organization of cells and their major organelles in weightlessness and hypergravity .
	manualset3
126551	9	405326	5	NULL	NULL	0	NULL	weightlessness 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-flight analysis included studies of cell formation , division rate , chemical composition , and ultrastructural organization of cells and their major organelles in weightlessness and hypergravity .
	manualset3
126552	10	405326	5	NULL	NULL	0	NULL	hypergravity 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-flight analysis included studies of cell formation , division rate , chemical composition , and ultrastructural organization of cells and their major organelles in weightlessness and hypergravity .
	manualset3
126553	1	405327	5	NULL	NULL	0	NULL	Post-mortem histopathological examination 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-mortem histopathological examination was consistent with dysautonomia .
	manualset3
126554	2	405327	5	NULL	NULL	0	NULL	dysautonomia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-mortem histopathological examination was consistent with dysautonomia .
	manualset3
126555	1	405328	5	NULL	NULL	0	NULL	Post-prandial endothelial dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-prandial endothelial dysfunction in hypertriglyceridemic subjects : molecular mechanisms and gene expression studies .
	manualset3
126556	2	405328	5	NULL	NULL	0	NULL	hypertriglyceridemic subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-prandial endothelial dysfunction in hypertriglyceridemic subjects : molecular mechanisms and gene expression studies .
	manualset3
126557	3	405328	5	NULL	NULL	0	NULL	molecular mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-prandial endothelial dysfunction in hypertriglyceridemic subjects : molecular mechanisms and gene expression studies .
	manualset3
126558	4	405328	5	NULL	NULL	0	NULL	gene expression studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-prandial endothelial dysfunction in hypertriglyceridemic subjects : molecular mechanisms and gene expression studies .
	manualset3
126559	1	405329	5	NULL	NULL	0	NULL	Post-thaw removal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-thaw removal of DMSO does not completely abrogate infusional toxicity or the need for pre-infusion histamine blockade .
	manualset3
126560	2	405329	5	NULL	NULL	0	NULL	DMSO 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-thaw removal of DMSO does not completely abrogate infusional toxicity or the need for pre-infusion histamine blockade .
	manualset3
126561	3	405329	5	NULL	NULL	0	NULL	infusional toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-thaw removal of DMSO does not completely abrogate infusional toxicity or the need for pre-infusion histamine blockade .
	manualset3
126562	4	405329	5	NULL	NULL	0	NULL	need	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-thaw removal of DMSO does not completely abrogate infusional toxicity or the need for pre-infusion histamine blockade .
	manualset3
126563	5	405329	5	NULL	NULL	0	NULL	pre-infusion histamine blockade	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-thaw removal of DMSO does not completely abrogate infusional toxicity or the need for pre-infusion histamine blockade .
	manualset3
126564	1	405330	5	NULL	NULL	0	NULL	 124 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A included 124 patients , 65 men and 59 women ( mean age 35 + / - 18 years ) , who reported frequent episodes of hypoglycemia ( HG ) .
	manualset3
126565	2	405330	5	NULL	NULL	0	NULL	 65 men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A included 124 patients , 65 men and 59 women ( mean age 35 + / - 18 years ) , who reported frequent episodes of hypoglycemia ( HG ) .
	manualset3
126566	3	405330	5	NULL	NULL	0	NULL	59 women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A included 124 patients , 65 men and 59 women ( mean age 35 + / - 18 years ) , who reported frequent episodes of hypoglycemia ( HG ) .
	manualset3
126567	4	405330	5	NULL	NULL	0	NULL	mean age 35 + / - 18 years	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A included 124 patients , 65 men and 59 women ( mean age 35 + / - 18 years ) , who reported frequent episodes of hypoglycemia ( HG ) .
	manualset3
126568	5	405330	5	NULL	NULL	0	NULL	frequent episodes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A included 124 patients , 65 men and 59 women ( mean age 35 + / - 18 years ) , who reported frequent episodes of hypoglycemia ( HG ) .
	manualset3
126569	6	405330	5	NULL	NULL	0	NULL	hypoglycemia ( HG )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A included 124 patients , 65 men and 59 women ( mean age 35 + / - 18 years ) , who reported frequent episodes of hypoglycemia ( HG ) .
	manualset3
128818	1	405331	5	NULL	NULL	0	NULL	Post-translational modifiers	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-translational modifiers of the small ubiquitin-like modifier protein ( SUMO ) family have emerged as key regulators of protein function and localization .
	manualset3
128819	2	405331	5	NULL	NULL	0	NULL	small ubiquitin-like modifier protein ( SUMO ) family 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-translational modifiers of the small ubiquitin-like modifier protein ( SUMO ) family have emerged as key regulators of protein function and localization .
	manualset3
128820	3	405331	5	NULL	NULL	0	NULL	key regulators	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-translational modifiers of the small ubiquitin-like modifier protein ( SUMO ) family have emerged as key regulators of protein function and localization .
	manualset3
128821	4	405331	5	NULL	NULL	0	NULL	protein function 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-translational modifiers of the small ubiquitin-like modifier protein ( SUMO ) family have emerged as key regulators of protein function and localization .
	manualset3
128822	5	405331	5	NULL	NULL	0	NULL	localization 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-translational modifiers of the small ubiquitin-like modifier protein ( SUMO ) family have emerged as key regulators of protein function and localization .
	manualset3
128823	1	405332	5	NULL	NULL	0	NULL	Post-translational regulatory mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-translational regulatory mechanisms ( e.g. , phosphorylation , nuclear translocation , multimerization , regulated degradation , etc. ) play particularly important roles because they enable cells to respond to various intra - and extracellular stimuli quickly and without prior protein synthesis .
	manualset3
128824	2	405332	5	NULL	NULL	0	NULL	phosphorylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-translational regulatory mechanisms ( e.g. , phosphorylation , nuclear translocation , multimerization , regulated degradation , etc. ) play particularly important roles because they enable cells to respond to various intra - and extracellular stimuli quickly and without prior protein synthesis .
	manualset3
128825	3	405332	5	NULL	NULL	0	NULL	nuclear translocation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-translational regulatory mechanisms ( e.g. , phosphorylation , nuclear translocation , multimerization , regulated degradation , etc. ) play particularly important roles because they enable cells to respond to various intra - and extracellular stimuli quickly and without prior protein synthesis .
	manualset3
128826	4	405332	5	NULL	NULL	0	NULL	multimerization 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-translational regulatory mechanisms ( e.g. , phosphorylation , nuclear translocation , multimerization , regulated degradation , etc. ) play particularly important roles because they enable cells to respond to various intra - and extracellular stimuli quickly and without prior protein synthesis .
	manualset3
128827	5	405332	5	NULL	NULL	0	NULL	regulated degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-translational regulatory mechanisms ( e.g. , phosphorylation , nuclear translocation , multimerization , regulated degradation , etc. ) play particularly important roles because they enable cells to respond to various intra - and extracellular stimuli quickly and without prior protein synthesis .
	manualset3
128828	6	405332	5	NULL	NULL	0	NULL	important roles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-translational regulatory mechanisms ( e.g. , phosphorylation , nuclear translocation , multimerization , regulated degradation , etc. ) play particularly important roles because they enable cells to respond to various intra - and extracellular stimuli quickly and without prior protein synthesis .
	manualset3
128829	7	405332	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-translational regulatory mechanisms ( e.g. , phosphorylation , nuclear translocation , multimerization , regulated degradation , etc. ) play particularly important roles because they enable cells to respond to various intra - and extracellular stimuli quickly and without prior protein synthesis .
	manualset3
128830	8	405332	5	NULL	NULL	0	NULL	respond 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-translational regulatory mechanisms ( e.g. , phosphorylation , nuclear translocation , multimerization , regulated degradation , etc. ) play particularly important roles because they enable cells to respond to various intra - and extracellular stimuli quickly and without prior protein synthesis .
	manualset3
128831	9	405332	5	NULL	NULL	0	NULL	intra - and extracellular stimuli 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-translational regulatory mechanisms ( e.g. , phosphorylation , nuclear translocation , multimerization , regulated degradation , etc. ) play particularly important roles because they enable cells to respond to various intra - and extracellular stimuli quickly and without prior protein synthesis .
	manualset3
128832	10	405332	5	NULL	NULL	0	NULL	prior protein synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-translational regulatory mechanisms ( e.g. , phosphorylation , nuclear translocation , multimerization , regulated degradation , etc. ) play particularly important roles because they enable cells to respond to various intra - and extracellular stimuli quickly and without prior protein synthesis .
	manualset3
128833	1	405333	5	NULL	NULL	0	NULL	Post-traumatic syndrome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-traumatic syndrome after minor head injury can not be predicted by neurological investigations .
	manualset3
128834	2	405333	5	NULL	NULL	0	NULL	minor head injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-traumatic syndrome after minor head injury can not be predicted by neurological investigations .
	manualset3
128835	3	405333	5	NULL	NULL	0	NULL	neurological investigations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-traumatic syndrome after minor head injury can not be predicted by neurological investigations .
	manualset3
128836	1	405334	5	NULL	NULL	NULL	NULL	Post-vaccination	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Post-vaccination , anti-pneumococcal IgG titers in group 1 were significantly lower than those in group 2 ( p = 0.012 for IgG post-vaccination and p = 0.020 for IgG2 post-vaccination ) .
	manualset3
128837	2	405334	5	NULL	NULL	0	NULL	anti-pneumococcal IgG titers	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-vaccination , anti-pneumococcal IgG titers in group 1 were significantly lower than those in group 2 ( p = 0.012 for IgG post-vaccination and p = 0.020 for IgG2 post-vaccination ) .
	manualset3
128838	3	405334	5	NULL	NULL	0	NULL	group 1 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-vaccination , anti-pneumococcal IgG titers in group 1 were significantly lower than those in group 2 ( p = 0.012 for IgG post-vaccination and p = 0.020 for IgG2 post-vaccination ) .
	manualset3
128839	4	405334	5	NULL	NULL	0	NULL	group 2	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-vaccination , anti-pneumococcal IgG titers in group 1 were significantly lower than those in group 2 ( p = 0.012 for IgG post-vaccination and p = 0.020 for IgG2 post-vaccination ) .
	manualset3
128840	5	405334	5	NULL	NULL	0	NULL	p = 0.012 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-vaccination , anti-pneumococcal IgG titers in group 1 were significantly lower than those in group 2 ( p = 0.012 for IgG post-vaccination and p = 0.020 for IgG2 post-vaccination ) .
	manualset3
128841	6	405334	5	NULL	NULL	0	NULL	IgG	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-vaccination , anti-pneumococcal IgG titers in group 1 were significantly lower than those in group 2 ( p = 0.012 for IgG post-vaccination and p = 0.020 for IgG2 post-vaccination ) .
	manualset3
128842	7	405334	5	NULL	NULL	NULL	NULL	post-vaccination	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Post-vaccination , anti-pneumococcal IgG titers in group 1 were significantly lower than those in group 2 ( p = 0.012 for IgG post-vaccination and p = 0.020 for IgG2 post-vaccination ) .
	manualset3
128843	8	405334	5	NULL	NULL	0	NULL	p = 0.020	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-vaccination , anti-pneumococcal IgG titers in group 1 were significantly lower than those in group 2 ( p = 0.012 for IgG post-vaccination and p = 0.020 for IgG2 post-vaccination ) .
	manualset3
128844	9	405334	5	NULL	NULL	0	NULL	IgG2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-vaccination , anti-pneumococcal IgG titers in group 1 were significantly lower than those in group 2 ( p = 0.012 for IgG post-vaccination and p = 0.020 for IgG2 post-vaccination ) .
	manualset3
128845	10	405334	5	NULL	NULL	0	NULL	post-vaccination	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Post-vaccination , anti-pneumococcal IgG titers in group 1 were significantly lower than those in group 2 ( p = 0.012 for IgG post-vaccination and p = 0.020 for IgG2 post-vaccination ) .
	manualset3
128846	1	405335	5	NULL	NULL	0	NULL	Postbinding function studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Postbinding function studies have shown a definite enhancement of peripheral glucose metabolism by sulfonylurea drugs ; such post-receptor changes have not clearly correlated with receptor binding alterations .
	manualset3
128847	2	405335	5	NULL	NULL	0	NULL	definite enhancement 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Postbinding function studies have shown a definite enhancement of peripheral glucose metabolism by sulfonylurea drugs ; such post-receptor changes have not clearly correlated with receptor binding alterations .
	manualset3
128848	3	405335	5	NULL	NULL	0	NULL	peripheral glucose metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Postbinding function studies have shown a definite enhancement of peripheral glucose metabolism by sulfonylurea drugs ; such post-receptor changes have not clearly correlated with receptor binding alterations .
	manualset3
128849	4	405335	5	NULL	NULL	0	NULL	sulfonylurea drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Postbinding function studies have shown a definite enhancement of peripheral glucose metabolism by sulfonylurea drugs ; such post-receptor changes have not clearly correlated with receptor binding alterations .
	manualset3
128850	5	405335	5	NULL	NULL	0	NULL	post-receptor changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Postbinding function studies have shown a definite enhancement of peripheral glucose metabolism by sulfonylurea drugs ; such post-receptor changes have not clearly correlated with receptor binding alterations .
	manualset3
128851	6	405335	5	NULL	NULL	0	NULL	receptor binding alterations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Postbinding function studies have shown a definite enhancement of peripheral glucose metabolism by sulfonylurea drugs ; such post-receptor changes have not clearly correlated with receptor binding alterations .
	manualset3
128852	1	405336	5	NULL	NULL	0	NULL	Posterior cruciate-retaining modular total knee arthroplasty	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Posterior cruciate-retaining modular total knee arthroplasty : a 9 - to 12-year follow-up investigation .
	manualset3
128853	2	405336	5	NULL	NULL	0	NULL	9 - to 12-year follow-up investigation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Posterior cruciate-retaining modular total knee arthroplasty : a 9 - to 12-year follow-up investigation .
	manualset3
128854	1	405337	5	NULL	NULL	0	NULL	Posterolateral decompression	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Posterolateral decompression and stabilization of thoracolumbar injuries using Diapason instrumentation .
	manualset3
128855	2	405337	5	NULL	NULL	0	NULL	stabilization 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Posterolateral decompression and stabilization of thoracolumbar injuries using Diapason instrumentation .
	manualset3
128856	3	405337	5	NULL	NULL	0	NULL	thoracolumbar injuries 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Posterolateral decompression and stabilization of thoracolumbar injuries using Diapason instrumentation .
	manualset3
128857	4	405337	5	NULL	NULL	0	NULL	Diapason instrumentation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Posterolateral decompression and stabilization of thoracolumbar injuries using Diapason instrumentation .
	manualset3
128858	1	405338	5	NULL	NULL	0	NULL	keratinocyte cell line expressing E7 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A keratinocyte cell line expressing E7 protein has been established and grafted onto syngeneic mice using a transplantation technique that permits the reformation of a differentiated epithelium on a granulation tissue bed .
	manualset3
128859	2	405338	5	NULL	NULL	0	NULL	syngeneic mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A keratinocyte cell line expressing E7 protein has been established and grafted onto syngeneic mice using a transplantation technique that permits the reformation of a differentiated epithelium on a granulation tissue bed .
	manualset3
128860	3	405338	5	NULL	NULL	0	NULL	transplantation technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A keratinocyte cell line expressing E7 protein has been established and grafted onto syngeneic mice using a transplantation technique that permits the reformation of a differentiated epithelium on a granulation tissue bed .
	manualset3
128861	4	405338	5	NULL	NULL	0	NULL	reformation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A keratinocyte cell line expressing E7 protein has been established and grafted onto syngeneic mice using a transplantation technique that permits the reformation of a differentiated epithelium on a granulation tissue bed .
	manualset3
128862	5	405338	5	NULL	NULL	0	NULL	differentiated epithelium	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	A keratinocyte cell line expressing E7 protein has been established and grafted onto syngeneic mice using a transplantation technique that permits the reformation of a differentiated epithelium on a granulation tissue bed .
	manualset3
128863	6	405338	5	NULL	NULL	0	NULL	granulation tissue bed 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	A keratinocyte cell line expressing E7 protein has been established and grafted onto syngeneic mice using a transplantation technique that permits the reformation of a differentiated epithelium on a granulation tissue bed .
	manualset3
128864	1	405339	5	NULL	NULL	0	NULL	Postmenopausal women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Postmenopausal women with established vertebral osteoporosis were studied for 2 years to determine the terminal elimination half-life and the duration of response to treatment with intravenous alendronate ( 30 mg ) given over 4 days .
	manualset3
128865	2	405339	5	NULL	NULL	0	NULL	vertebral osteoporosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Postmenopausal women with established vertebral osteoporosis were studied for 2 years to determine the terminal elimination half-life and the duration of response to treatment with intravenous alendronate ( 30 mg ) given over 4 days .
	manualset3
128866	3	405339	5	NULL	NULL	0	NULL	2 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Postmenopausal women with established vertebral osteoporosis were studied for 2 years to determine the terminal elimination half-life and the duration of response to treatment with intravenous alendronate ( 30 mg ) given over 4 days .
	manualset3
128867	4	405339	5	NULL	NULL	NULL	NULL	terminal elimination half-life	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Postmenopausal women with established vertebral osteoporosis were studied for 2 years to determine the terminal elimination half-life and the duration of response to treatment with intravenous alendronate ( 30 mg ) given over 4 days .
	manualset3
128868	5	405339	5	NULL	NULL	NULL	NULL	duration of response 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Postmenopausal women with established vertebral osteoporosis were studied for 2 years to determine the terminal elimination half-life and the duration of response to treatment with intravenous alendronate ( 30 mg ) given over 4 days .
	manualset3
128869	6	405339	5	NULL	NULL	0	NULL	treatment 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Postmenopausal women with established vertebral osteoporosis were studied for 2 years to determine the terminal elimination half-life and the duration of response to treatment with intravenous alendronate ( 30 mg ) given over 4 days .
	manualset3
128870	7	405339	5	NULL	NULL	0	NULL	intravenous alendronate	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Postmenopausal women with established vertebral osteoporosis were studied for 2 years to determine the terminal elimination half-life and the duration of response to treatment with intravenous alendronate ( 30 mg ) given over 4 days .
	manualset3
128871	8	405339	5	NULL	NULL	0	NULL	 30 mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Postmenopausal women with established vertebral osteoporosis were studied for 2 years to determine the terminal elimination half-life and the duration of response to treatment with intravenous alendronate ( 30 mg ) given over 4 days .
	manualset3
128872	9	405339	5	NULL	NULL	0	NULL	4 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Postmenopausal women with established vertebral osteoporosis were studied for 2 years to determine the terminal elimination half-life and the duration of response to treatment with intravenous alendronate ( 30 mg ) given over 4 days .
	manualset3
128873	1	405340	5	NULL	NULL	0	NULL	Postmodernism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Postmodernism is a philosophical and social movement which stresses that ideas are temporary , research data should be considered only in context , reality is transcendent , grand theories are invalid , problems are deconstructed , and findings should have practical value .
	manualset3
128874	2	405340	5	NULL	NULL	0	NULL	philosophical movement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Postmodernism is a philosophical and social movement which stresses that ideas are temporary , research data should be considered only in context , reality is transcendent , grand theories are invalid , problems are deconstructed , and findings should have practical value .
	manualset3
128875	3	405340	5	NULL	NULL	0	NULL	social movement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Postmodernism is a philosophical and social movement which stresses that ideas are temporary , research data should be considered only in context , reality is transcendent , grand theories are invalid , problems are deconstructed , and findings should have practical value .
	manualset3
128876	4	405340	5	NULL	NULL	0	NULL	ideas 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Postmodernism is a philosophical and social movement which stresses that ideas are temporary , research data should be considered only in context , reality is transcendent , grand theories are invalid , problems are deconstructed , and findings should have practical value .
	manualset3
128877	5	405340	5	NULL	NULL	0	NULL	research data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Postmodernism is a philosophical and social movement which stresses that ideas are temporary , research data should be considered only in context , reality is transcendent , grand theories are invalid , problems are deconstructed , and findings should have practical value .
	manualset3
128878	6	405340	5	NULL	NULL	0	NULL	context 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Postmodernism is a philosophical and social movement which stresses that ideas are temporary , research data should be considered only in context , reality is transcendent , grand theories are invalid , problems are deconstructed , and findings should have practical value .
	manualset3
128879	7	405340	5	NULL	NULL	0	NULL	reality 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Postmodernism is a philosophical and social movement which stresses that ideas are temporary , research data should be considered only in context , reality is transcendent , grand theories are invalid , problems are deconstructed , and findings should have practical value .
	manualset3
128880	8	405340	5	NULL	NULL	0	NULL	grand theories	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Postmodernism is a philosophical and social movement which stresses that ideas are temporary , research data should be considered only in context , reality is transcendent , grand theories are invalid , problems are deconstructed , and findings should have practical value .
	manualset3
128881	9	405340	5	NULL	NULL	0	NULL	problems 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Postmodernism is a philosophical and social movement which stresses that ideas are temporary , research data should be considered only in context , reality is transcendent , grand theories are invalid , problems are deconstructed , and findings should have practical value .
	manualset3
128882	10	405340	5	NULL	NULL	0	NULL	findings 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Postmodernism is a philosophical and social movement which stresses that ideas are temporary , research data should be considered only in context , reality is transcendent , grand theories are invalid , problems are deconstructed , and findings should have practical value .
	manualset3
128883	11	405340	5	NULL	NULL	0	NULL	practical value	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Postmodernism is a philosophical and social movement which stresses that ideas are temporary , research data should be considered only in context , reality is transcendent , grand theories are invalid , problems are deconstructed , and findings should have practical value .
	manualset3
128884	1	405341	5	NULL	NULL	0	NULL	Postnatal catch-up growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Postnatal catch-up growth in infants born small for gestational age has been reported to occur mainly during the initial 3-9 months of life .
	manualset3
128885	2	405341	5	NULL	NULL	0	NULL	infants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Postnatal catch-up growth in infants born small for gestational age has been reported to occur mainly during the initial 3-9 months of life .
	manualset3
128886	3	405341	5	NULL	NULL	0	NULL	gestational age	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Postnatal catch-up growth in infants born small for gestational age has been reported to occur mainly during the initial 3-9 months of life .
	manualset3
128887	4	405341	5	NULL	NULL	0	NULL	3-9 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Postnatal catch-up growth in infants born small for gestational age has been reported to occur mainly during the initial 3-9 months of life .
	manualset3
128888	5	405341	5	NULL	NULL	0	NULL	life 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Postnatal catch-up growth in infants born small for gestational age has been reported to occur mainly during the initial 3-9 months of life .
	manualset3
128893	1	405342	5	NULL	NULL	0	NULL	Postoperative bleeding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative bleeding into drains was marginally greater in the indomethacin group , although the difference was not statistically significant .
	manualset3
128894	2	405342	5	NULL	NULL	0	NULL	drains	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative bleeding into drains was marginally greater in the indomethacin group , although the difference was not statistically significant .
	manualset3
128895	3	405342	5	NULL	NULL	0	NULL	indomethacin group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative bleeding into drains was marginally greater in the indomethacin group , although the difference was not statistically significant .
	manualset3
128896	4	405342	5	NULL	NULL	0	NULL	difference	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative bleeding into drains was marginally greater in the indomethacin group , although the difference was not statistically significant .
	manualset3
128897	1	405343	5	NULL	NULL	0	NULL	Postoperative changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative changes in the breast may mimic a malignancy ; therefore , it is important to obtain an accurate history as to the timing of biopsy or surgery and to follow the changes in lesion morphology over time .
	manualset3
128898	2	405343	5	NULL	NULL	0	NULL	breast	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative changes in the breast may mimic a malignancy ; therefore , it is important to obtain an accurate history as to the timing of biopsy or surgery and to follow the changes in lesion morphology over time .
	manualset3
128899	3	405343	5	NULL	NULL	0	NULL	malignancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative changes in the breast may mimic a malignancy ; therefore , it is important to obtain an accurate history as to the timing of biopsy or surgery and to follow the changes in lesion morphology over time .
	manualset3
128900	4	405343	5	NULL	NULL	0	NULL	accurate history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative changes in the breast may mimic a malignancy ; therefore , it is important to obtain an accurate history as to the timing of biopsy or surgery and to follow the changes in lesion morphology over time .
	manualset3
128901	5	405343	5	NULL	NULL	0	NULL	timing	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative changes in the breast may mimic a malignancy ; therefore , it is important to obtain an accurate history as to the timing of biopsy or surgery and to follow the changes in lesion morphology over time .
	manualset3
128902	6	405343	5	NULL	NULL	0	NULL	biopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative changes in the breast may mimic a malignancy ; therefore , it is important to obtain an accurate history as to the timing of biopsy or surgery and to follow the changes in lesion morphology over time .
	manualset3
128903	7	405343	5	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative changes in the breast may mimic a malignancy ; therefore , it is important to obtain an accurate history as to the timing of biopsy or surgery and to follow the changes in lesion morphology over time .
	manualset3
128904	8	405343	5	NULL	NULL	NULL	NULL	lesion morphology	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Postoperative changes in the breast may mimic a malignancy ; therefore , it is important to obtain an accurate history as to the timing of biopsy or surgery and to follow the changes in lesion morphology over time .
	manualset3
128905	9	405343	5	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative changes in the breast may mimic a malignancy ; therefore , it is important to obtain an accurate history as to the timing of biopsy or surgery and to follow the changes in lesion morphology over time .
	manualset3
134848	10	405343	5	NULL	NULL	0	NULL	changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative changes in the breast may mimic a malignancy ; therefore , it is important to obtain an accurate history as to the timing of biopsy or surgery and to follow the changes in lesion morphology over time .
	manualset3
128906	1	405344	5	NULL	NULL	0	NULL	Postoperative follow-up	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative follow-up may be regarded as the screening of a high-risk group .
	manualset3
128907	2	405344	5	NULL	NULL	0	NULL	screening	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative follow-up may be regarded as the screening of a high-risk group .
	manualset3
128908	3	405344	5	NULL	NULL	0	NULL	high-risk group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative follow-up may be regarded as the screening of a high-risk group .
	manualset3
128909	1	405345	5	NULL	NULL	0	NULL	Postoperative follow-up time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative follow-up time ranged from three to 24 months , with 82 patients having at least one year of follow-up .
	manualset3
128910	2	405345	5	NULL	NULL	0	NULL	three to 24 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative follow-up time ranged from three to 24 months , with 82 patients having at least one year of follow-up .
	manualset3
128911	3	405345	5	NULL	NULL	0	NULL	82 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative follow-up time ranged from three to 24 months , with 82 patients having at least one year of follow-up .
	manualset3
128912	4	405345	5	NULL	NULL	0	NULL	one year	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative follow-up time ranged from three to 24 months , with 82 patients having at least one year of follow-up .
	manualset3
128913	5	405345	5	NULL	NULL	0	NULL	follow-up	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative follow-up time ranged from three to 24 months , with 82 patients having at least one year of follow-up .
	manualset3
128914	1	405346	5	NULL	NULL	0	NULL	Postoperative opisthotonus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative opisthotonus and torticollis after fentanyl , enflurane , and nitrous oxide .
	manualset3
128915	2	405346	5	NULL	NULL	0	NULL	torticollis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative opisthotonus and torticollis after fentanyl , enflurane , and nitrous oxide .
	manualset3
128916	3	405346	5	NULL	NULL	0	NULL	fentanyl	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative opisthotonus and torticollis after fentanyl , enflurane , and nitrous oxide .
	manualset3
128917	4	405346	5	NULL	NULL	0	NULL	enflurane	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative opisthotonus and torticollis after fentanyl , enflurane , and nitrous oxide .
	manualset3
128918	5	405346	5	NULL	NULL	0	NULL	nitrous oxide	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative opisthotonus and torticollis after fentanyl , enflurane , and nitrous oxide .
	manualset3
128919	1	405347	5	NULL	NULL	0	NULL	key diagnostic requisite	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A key diagnostic requisite is the absence of organic , metabolic , or systemic disorders to explain `` dyspeptic symptoms . ''
	manualset3
128920	2	405347	5	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A key diagnostic requisite is the absence of organic , metabolic , or systemic disorders to explain `` dyspeptic symptoms . ''
	manualset3
128921	3	405347	5	NULL	NULL	NULL	NULL	organic disorders	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A key diagnostic requisite is the absence of organic , metabolic , or systemic disorders to explain `` dyspeptic symptoms . ''
	manualset3
128922	6	405347	5	NULL	NULL	NULL	NULL	dyspeptic symptoms	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A key diagnostic requisite is the absence of organic , metabolic , or systemic disorders to explain `` dyspeptic symptoms . ''
	manualset3
134849	4	405347	5	NULL	NULL	NULL	NULL	metabolic disorders	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A key diagnostic requisite is the absence of organic , metabolic , or systemic disorders to explain `` dyspeptic symptoms . ''
	manualset3
134850	5	405347	5	NULL	NULL	0	NULL	systemic disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A key diagnostic requisite is the absence of organic , metabolic , or systemic disorders to explain `` dyspeptic symptoms . ''
	manualset3
128923	1	405348	5	NULL	NULL	0	NULL	Postoperative pulmonary complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative pulmonary complications occurred in 20 cases ( 36 % ) ; pneumonia in 7 cases ( 13 % ) , lung edema in 12 cases ( 22 % ) , atelectasis in one case ( 2 % ) .
	manualset3
128924	2	405348	5	NULL	NULL	0	NULL	20 cases	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative pulmonary complications occurred in 20 cases ( 36 % ) ; pneumonia in 7 cases ( 13 % ) , lung edema in 12 cases ( 22 % ) , atelectasis in one case ( 2 % ) .
	manualset3
128925	3	405348	5	NULL	NULL	0	NULL	36 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative pulmonary complications occurred in 20 cases ( 36 % ) ; pneumonia in 7 cases ( 13 % ) , lung edema in 12 cases ( 22 % ) , atelectasis in one case ( 2 % ) .
	manualset3
128926	4	405348	5	NULL	NULL	0	NULL	pneumonia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative pulmonary complications occurred in 20 cases ( 36 % ) ; pneumonia in 7 cases ( 13 % ) , lung edema in 12 cases ( 22 % ) , atelectasis in one case ( 2 % ) .
	manualset3
128927	5	405348	5	NULL	NULL	0	NULL	7 cases	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative pulmonary complications occurred in 20 cases ( 36 % ) ; pneumonia in 7 cases ( 13 % ) , lung edema in 12 cases ( 22 % ) , atelectasis in one case ( 2 % ) .
	manualset3
128928	6	405348	5	NULL	NULL	0	NULL	13 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative pulmonary complications occurred in 20 cases ( 36 % ) ; pneumonia in 7 cases ( 13 % ) , lung edema in 12 cases ( 22 % ) , atelectasis in one case ( 2 % ) .
	manualset3
128929	7	405348	5	NULL	NULL	0	NULL	lung edema	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative pulmonary complications occurred in 20 cases ( 36 % ) ; pneumonia in 7 cases ( 13 % ) , lung edema in 12 cases ( 22 % ) , atelectasis in one case ( 2 % ) .
	manualset3
128930	8	405348	5	NULL	NULL	0	NULL	12 cases	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative pulmonary complications occurred in 20 cases ( 36 % ) ; pneumonia in 7 cases ( 13 % ) , lung edema in 12 cases ( 22 % ) , atelectasis in one case ( 2 % ) .
	manualset3
128931	9	405348	5	NULL	NULL	0	NULL	22 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative pulmonary complications occurred in 20 cases ( 36 % ) ; pneumonia in 7 cases ( 13 % ) , lung edema in 12 cases ( 22 % ) , atelectasis in one case ( 2 % ) .
	manualset3
128932	10	405348	5	NULL	NULL	0	NULL	atelectasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative pulmonary complications occurred in 20 cases ( 36 % ) ; pneumonia in 7 cases ( 13 % ) , lung edema in 12 cases ( 22 % ) , atelectasis in one case ( 2 % ) .
	manualset3
128933	11	405348	5	NULL	NULL	0	NULL	one case	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative pulmonary complications occurred in 20 cases ( 36 % ) ; pneumonia in 7 cases ( 13 % ) , lung edema in 12 cases ( 22 % ) , atelectasis in one case ( 2 % ) .
	manualset3
128934	12	405348	5	NULL	NULL	0	NULL	2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative pulmonary complications occurred in 20 cases ( 36 % ) ; pneumonia in 7 cases ( 13 % ) , lung edema in 12 cases ( 22 % ) , atelectasis in one case ( 2 % ) .
	manualset3
128935	1	405349	5	NULL	NULL	0	NULL	Postoperative visual loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative visual loss associated with spine surgery is a rare complication with no established definitive etiology .
	manualset3
128936	2	405349	5	NULL	NULL	0	NULL	spine surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative visual loss associated with spine surgery is a rare complication with no established definitive etiology .
	manualset3
128937	3	405349	5	NULL	NULL	0	NULL	rare complication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative visual loss associated with spine surgery is a rare complication with no established definitive etiology .
	manualset3
128938	4	405349	5	NULL	NULL	0	NULL	definitive etiology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative visual loss associated with spine surgery is a rare complication with no established definitive etiology .
	manualset3
128939	1	405350	5	NULL	NULL	0	NULL	endocrine levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperatively , endocrine levels and distress were not clearly related .
	manualset3
128940	2	405350	5	NULL	NULL	0	NULL	distress 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperatively , endocrine levels and distress were not clearly related .
	manualset3
128941	1	405351	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperatively , patients were evaluated for pain scores and the total doses of meperidine required over 24 hours .
	manualset3
128942	2	405351	5	NULL	NULL	0	NULL	pain scores 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperatively , patients were evaluated for pain scores and the total doses of meperidine required over 24 hours .
	manualset3
128943	3	405351	5	NULL	NULL	0	NULL	total doses 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperatively , patients were evaluated for pain scores and the total doses of meperidine required over 24 hours .
	manualset3
128944	4	405351	5	NULL	NULL	0	NULL	meperidine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperatively , patients were evaluated for pain scores and the total doses of meperidine required over 24 hours .
	manualset3
128945	5	405351	5	NULL	NULL	0	NULL	24 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperatively , patients were evaluated for pain scores and the total doses of meperidine required over 24 hours .
	manualset3
128946	1	405352	5	NULL	NULL	0	NULL	Postprandial effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Postprandial effects of feeding triglycerides or their digestion products on the quantity and fatty acid pattern of the major serum lipid classes .
	manualset3
128947	2	405352	5	NULL	NULL	0	NULL	triglycerides 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Postprandial effects of feeding triglycerides or their digestion products on the quantity and fatty acid pattern of the major serum lipid classes .
	manualset3
128948	3	405352	5	NULL	NULL	0	NULL	digestion products	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Postprandial effects of feeding triglycerides or their digestion products on the quantity and fatty acid pattern of the major serum lipid classes .
	manualset3
128949	4	405352	5	NULL	NULL	0	NULL	quantity 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Postprandial effects of feeding triglycerides or their digestion products on the quantity and fatty acid pattern of the major serum lipid classes .
	manualset3
128950	5	405352	5	NULL	NULL	0	NULL	fatty acid pattern	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Postprandial effects of feeding triglycerides or their digestion products on the quantity and fatty acid pattern of the major serum lipid classes .
	manualset3
128951	6	405352	5	NULL	NULL	0	NULL	major serum lipid classes	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Postprandial effects of feeding triglycerides or their digestion products on the quantity and fatty acid pattern of the major serum lipid classes .
	manualset3
128952	1	405353	5	NULL	NULL	0	NULL	Postprandial platelet-poor plasma 5-hydroxytryptamine concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Postprandial platelet-poor plasma 5-hydroxytryptamine concentrations during diarrhea and constipation periods of alternatingtype irritable bowel syndrome patients .
	manualset3
128953	2	405353	5	NULL	NULL	0	NULL	diarrhea 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Postprandial platelet-poor plasma 5-hydroxytryptamine concentrations during diarrhea and constipation periods of alternatingtype irritable bowel syndrome patients .
	manualset3
128954	3	405353	5	NULL	NULL	0	NULL	constipation periods	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Postprandial platelet-poor plasma 5-hydroxytryptamine concentrations during diarrhea and constipation periods of alternatingtype irritable bowel syndrome patients .
	manualset3
128955	4	405353	5	NULL	NULL	0	NULL	alternatingtype irritable bowel syndrome patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Postprandial platelet-poor plasma 5-hydroxytryptamine concentrations during diarrhea and constipation periods of alternatingtype irritable bowel syndrome patients .
	manualset3
128956	1	405354	5	NULL	NULL	0	NULL	Postprocedural mean pressure gradient 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Postprocedural mean pressure gradient across the mitral valve decreased to 6mmHg from an initially recorded value of 22mmHg .
	manualset3
128957	2	405354	5	NULL	NULL	0	NULL	mitral valve	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Postprocedural mean pressure gradient across the mitral valve decreased to 6mmHg from an initially recorded value of 22mmHg .
	manualset3
128958	3	405354	5	NULL	NULL	0	NULL	 6mmHg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Postprocedural mean pressure gradient across the mitral valve decreased to 6mmHg from an initially recorded value of 22mmHg .
	manualset3
128959	4	405354	5	NULL	NULL	0	NULL	initially recorded value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Postprocedural mean pressure gradient across the mitral valve decreased to 6mmHg from an initially recorded value of 22mmHg .
	manualset3
128960	5	405354	5	NULL	NULL	0	NULL	 22mmHg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Postprocedural mean pressure gradient across the mitral valve decreased to 6mmHg from an initially recorded value of 22mmHg .
	manualset3
128961	1	405355	5	NULL	NULL	0	NULL	Postsynaptic doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Postsynaptic doses of apomorphine administered to acutely tested rats induced more scanning with , and more turning toward , the intact vibrissae side .
	manualset3
128962	2	405355	5	NULL	NULL	0	NULL	apomorphine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Postsynaptic doses of apomorphine administered to acutely tested rats induced more scanning with , and more turning toward , the intact vibrissae side .
	manualset3
128963	3	405355	5	NULL	NULL	0	NULL	acutely tested rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Postsynaptic doses of apomorphine administered to acutely tested rats induced more scanning with , and more turning toward , the intact vibrissae side .
	manualset3
128964	4	405355	5	NULL	NULL	0	NULL	intact vibrissae side	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Postsynaptic doses of apomorphine administered to acutely tested rats induced more scanning with , and more turning toward , the intact vibrissae side .
	manualset3
128965	1	405356	5	NULL	NULL	0	NULL	Postsynaptic potential generation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Postsynaptic potential generation appears independent of synaptic elevation of cyclic nucleotides in sympathetic neurons .
	manualset3
128966	2	405356	5	NULL	NULL	0	NULL	synaptic elevation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Postsynaptic potential generation appears independent of synaptic elevation of cyclic nucleotides in sympathetic neurons .
	manualset3
128967	3	405356	5	NULL	NULL	0	NULL	cyclic nucleotides	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Postsynaptic potential generation appears independent of synaptic elevation of cyclic nucleotides in sympathetic neurons .
	manualset3
128968	4	405356	5	NULL	NULL	0	NULL	sympathetic neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Postsynaptic potential generation appears independent of synaptic elevation of cyclic nucleotides in sympathetic neurons .
	manualset3
128969	1	405357	5	NULL	NULL	0	NULL	Posttraumatic administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Posttraumatic administration of bFGF significantly reduced the numbers of damaged cortical neuron profiles at several coronal levels and reduced the total number of damaged neurons ( 696 + / - 148 vs. 1 , 248 + / - 198 , means + / - SEM ) , p & lt ; 0.05 , ANOVA ) .
	manualset3
128970	2	405357	5	NULL	NULL	0	NULL	bFGF 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Posttraumatic administration of bFGF significantly reduced the numbers of damaged cortical neuron profiles at several coronal levels and reduced the total number of damaged neurons ( 696 + / - 148 vs. 1 , 248 + / - 198 , means + / - SEM ) , p & lt ; 0.05 , ANOVA ) .
	manualset3
128971	3	405357	5	NULL	NULL	0	NULL	numbers 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Posttraumatic administration of bFGF significantly reduced the numbers of damaged cortical neuron profiles at several coronal levels and reduced the total number of damaged neurons ( 696 + / - 148 vs. 1 , 248 + / - 198 , means + / - SEM ) , p & lt ; 0.05 , ANOVA ) .
	manualset3
128972	4	405357	5	NULL	NULL	0	NULL	damaged cortical neuron profiles	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Posttraumatic administration of bFGF significantly reduced the numbers of damaged cortical neuron profiles at several coronal levels and reduced the total number of damaged neurons ( 696 + / - 148 vs. 1 , 248 + / - 198 , means + / - SEM ) , p & lt ; 0.05 , ANOVA ) .
	manualset3
128973	5	405357	5	NULL	NULL	0	NULL	coronal levels	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Posttraumatic administration of bFGF significantly reduced the numbers of damaged cortical neuron profiles at several coronal levels and reduced the total number of damaged neurons ( 696 + / - 148 vs. 1 , 248 + / - 198 , means + / - SEM ) , p & lt ; 0.05 , ANOVA ) .
	manualset3
128974	6	405357	5	NULL	NULL	0	NULL	total number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Posttraumatic administration of bFGF significantly reduced the numbers of damaged cortical neuron profiles at several coronal levels and reduced the total number of damaged neurons ( 696 + / - 148 vs. 1 , 248 + / - 198 , means + / - SEM ) , p & lt ; 0.05 , ANOVA ) .
	manualset3
128975	7	405357	5	NULL	NULL	0	NULL	damaged neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Posttraumatic administration of bFGF significantly reduced the numbers of damaged cortical neuron profiles at several coronal levels and reduced the total number of damaged neurons ( 696 + / - 148 vs. 1 , 248 + / - 198 , means + / - SEM ) , p & lt ; 0.05 , ANOVA ) .
	manualset3
128976	8	405357	5	NULL	NULL	0	NULL	696 + / - 148 vs. 1 , 248 + / - 198 , means + / - SEM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Posttraumatic administration of bFGF significantly reduced the numbers of damaged cortical neuron profiles at several coronal levels and reduced the total number of damaged neurons ( 696 + / - 148 vs. 1 , 248 + / - 198 , means + / - SEM ) , p & lt ; 0.05 , ANOVA ) .
	manualset3
128977	9	405357	5	NULL	NULL	0	NULL	 p & lt ; 0.05 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Posttraumatic administration of bFGF significantly reduced the numbers of damaged cortical neuron profiles at several coronal levels and reduced the total number of damaged neurons ( 696 + / - 148 vs. 1 , 248 + / - 198 , means + / - SEM ) , p & lt ; 0.05 , ANOVA ) .
	manualset3
128978	10	405357	5	NULL	NULL	0	NULL	ANOVA 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Posttraumatic administration of bFGF significantly reduced the numbers of damaged cortical neuron profiles at several coronal levels and reduced the total number of damaged neurons ( 696 + / - 148 vs. 1 , 248 + / - 198 , means + / - SEM ) , p & lt ; 0.05 , ANOVA ) .
	manualset3
128979	1	405358	5	NULL	NULL	0	NULL	Posttraumatic stress symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Posttraumatic stress symptoms and medical procedures in children .
	manualset3
128980	2	405358	5	NULL	NULL	0	NULL	medical procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Posttraumatic stress symptoms and medical procedures in children .
	manualset3
128981	3	405358	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Posttraumatic stress symptoms and medical procedures in children .
	manualset3
128982	1	405359	5	NULL	NULL	0	NULL	Postural hypotension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Postural hypotension can be particularly troublesome in the elderly .
	manualset3
128983	2	405359	5	NULL	NULL	0	NULL	elderly 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Postural hypotension can be particularly troublesome in the elderly .
	manualset3
128984	1	405360	5	NULL	NULL	0	NULL	Postural sway ( i.e. , center-of-pressure ) dynamics	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Postural sway ( i.e. , center-of-pressure ) dynamics were assessed during quiet standing and cognitive dual tasking , and a complexity index was quantified using multiscale entropy analysis .
	manualset3
128985	2	405360	5	NULL	NULL	0	NULL	quiet standing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Postural sway ( i.e. , center-of-pressure ) dynamics were assessed during quiet standing and cognitive dual tasking , and a complexity index was quantified using multiscale entropy analysis .
	manualset3
128986	3	405360	5	NULL	NULL	0	NULL	cognitive dual tasking	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Postural sway ( i.e. , center-of-pressure ) dynamics were assessed during quiet standing and cognitive dual tasking , and a complexity index was quantified using multiscale entropy analysis .
	manualset3
128987	4	405360	5	NULL	NULL	0	NULL	complexity index 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Postural sway ( i.e. , center-of-pressure ) dynamics were assessed during quiet standing and cognitive dual tasking , and a complexity index was quantified using multiscale entropy analysis .
	manualset3
128988	5	405360	5	NULL	NULL	0	NULL	multiscale entropy analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Postural sway ( i.e. , center-of-pressure ) dynamics were assessed during quiet standing and cognitive dual tasking , and a complexity index was quantified using multiscale entropy analysis .
	manualset3
128989	1	405361	5	NULL	NULL	0	NULL	Potassium 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Potassium and its effect on glycogen in the dog heart .
	manualset3
128990	2	405361	5	NULL	NULL	0	NULL	glycogen 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Potassium and its effect on glycogen in the dog heart .
	manualset3
128991	3	405361	5	NULL	NULL	0	NULL	dog heart	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Potassium and its effect on glycogen in the dog heart .
	manualset3
128992	1	405362	5	NULL	NULL	NULL	NULL	Potassium channels	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Potassium channels : structures , models , simulations .
	manualset3
128993	2	405362	5	NULL	NULL	0	NULL	structures 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Potassium channels : structures , models , simulations .
	manualset3
128994	3	405362	5	NULL	NULL	0	NULL	models 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Potassium channels : structures , models , simulations .
	manualset3
128995	4	405362	5	NULL	NULL	0	NULL	simulations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Potassium channels : structures , models , simulations .
	manualset3
128996	1	405363	5	NULL	NULL	0	NULL	Potassium deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Potassium deficiency causes depletion of intracellular potassium and increased intracellular accumulation of basic amino acids .
	manualset3
128997	2	405363	5	NULL	NULL	0	NULL	depletion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Potassium deficiency causes depletion of intracellular potassium and increased intracellular accumulation of basic amino acids .
	manualset3
128998	3	405363	5	NULL	NULL	0	NULL	intracellular potassium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Potassium deficiency causes depletion of intracellular potassium and increased intracellular accumulation of basic amino acids .
	manualset3
128999	4	405363	5	NULL	NULL	0	NULL	intracellular accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Potassium deficiency causes depletion of intracellular potassium and increased intracellular accumulation of basic amino acids .
	manualset3
129000	5	405363	5	NULL	NULL	0	NULL	basic amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Potassium deficiency causes depletion of intracellular potassium and increased intracellular accumulation of basic amino acids .
	manualset3
129001	1	405364	5	NULL	NULL	0	NULL	Potassium scandium niobate hydroxide, K(3)(Sc(0.875)Nb(0.125))Nb(2)O(9)H(1.75)	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Potassium scandium niobate hydroxide , K ( 3 ) ( Sc ( 0.875 ) Nb ( 0.125 ) ) Nb ( 2 ) O ( 9 ) H ( 1.75 ) , is a new scandium niobate with a unique cage structure .
	manualset3
129002	2	405364	5	NULL	NULL	0	NULL	scandium niobate	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Potassium scandium niobate hydroxide , K ( 3 ) ( Sc ( 0.875 ) Nb ( 0.125 ) ) Nb ( 2 ) O ( 9 ) H ( 1.75 ) , is a new scandium niobate with a unique cage structure .
	manualset3
129003	3	405364	5	NULL	NULL	0	NULL	unique cage structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Potassium scandium niobate hydroxide , K ( 3 ) ( Sc ( 0.875 ) Nb ( 0.125 ) ) Nb ( 2 ) O ( 9 ) H ( 1.75 ) , is a new scandium niobate with a unique cage structure .
	manualset3
129004	1	405365	5	NULL	NULL	0	NULL	Calcium 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	( Calcium and folic acid are delicate knotty questions ) .
	manualset3
129005	2	405365	5	NULL	NULL	0	NULL	folic acid 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	( Calcium and folic acid are delicate knotty questions ) .
	manualset3
134851	3	405365	5	NULL	NULL	NULL	NULL	knotty questions	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Calcium and folic acid are delicate knotty questions ) .
	manualset3
129006	1	405366	5	NULL	NULL	0	NULL	laboratory investigation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A laboratory investigation of tunnel restorations in premolar teeth .
	manualset3
129007	2	405366	5	NULL	NULL	0	NULL	tunnel restorations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A laboratory investigation of tunnel restorations in premolar teeth .
	manualset3
129008	3	405366	5	NULL	NULL	0	NULL	premolar teeth	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A laboratory investigation of tunnel restorations in premolar teeth .
	manualset3
129009	1	405367	5	NULL	NULL	0	NULL	Potent thyrotrophin receptor-blocking antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Potent thyrotrophin receptor-blocking antibodies : a cause of transient congenital hypothyroidism and delayed thyroid development .
	manualset3
129010	2	405367	5	NULL	NULL	0	NULL	transient congenital hypothyroidism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Potent thyrotrophin receptor-blocking antibodies : a cause of transient congenital hypothyroidism and delayed thyroid development .
	manualset3
129011	3	405367	5	NULL	NULL	0	NULL	delayed thyroid development	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Potent thyrotrophin receptor-blocking antibodies : a cause of transient congenital hypothyroidism and delayed thyroid development .
	manualset3
134852	4	405367	5	NULL	NULL	0	NULL	cause	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Potent thyrotrophin receptor-blocking antibodies : a cause of transient congenital hypothyroidism and delayed thyroid development .
	manualset3
129012	1	405368	5	NULL	NULL	0	NULL	Potential alternate transport destinations 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential alternate transport destinations include physician office buildings , ambulatory care centers , ambulatory surgery centers , and urgent care centers .
	manualset3
129013	2	405368	5	NULL	NULL	0	NULL	physician office buildings	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential alternate transport destinations include physician office buildings , ambulatory care centers , ambulatory surgery centers , and urgent care centers .
	manualset3
129014	3	405368	5	NULL	NULL	0	NULL	ambulatory care centers	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential alternate transport destinations include physician office buildings , ambulatory care centers , ambulatory surgery centers , and urgent care centers .
	manualset3
129015	4	405368	5	NULL	NULL	0	NULL	ambulatory surgery centers	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential alternate transport destinations include physician office buildings , ambulatory care centers , ambulatory surgery centers , and urgent care centers .
	manualset3
129016	5	405368	5	NULL	NULL	0	NULL	urgent care centers	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential alternate transport destinations include physician office buildings , ambulatory care centers , ambulatory surgery centers , and urgent care centers .
	manualset3
129017	1	405369	5	NULL	NULL	0	NULL	Potential applications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential applications include affine invariant image segmentation , registration , affine symmetric image coding , and motion analysis .
	manualset3
129018	2	405369	5	NULL	NULL	0	NULL	affine invariant image segmentation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential applications include affine invariant image segmentation , registration , affine symmetric image coding , and motion analysis .
	manualset3
129019	3	405369	5	NULL	NULL	0	NULL	registration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential applications include affine invariant image segmentation , registration , affine symmetric image coding , and motion analysis .
	manualset3
129020	4	405369	5	NULL	NULL	0	NULL	affine symmetric image coding	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential applications include affine invariant image segmentation , registration , affine symmetric image coding , and motion analysis .
	manualset3
129021	5	405369	5	NULL	NULL	0	NULL	motion analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential applications include affine invariant image segmentation , registration , affine symmetric image coding , and motion analysis .
	manualset3
129022	1	405370	5	NULL	NULL	0	NULL	deficits in olfaction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential causes including deficits in olfaction and lactation were not apparent .
	manualset3
129023	2	405370	5	NULL	NULL	0	NULL	deficits in lactation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential causes including deficits in olfaction and lactation were not apparent .
	manualset3
134853	3	405370	5	NULL	NULL	0	NULL	causes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential causes including deficits in olfaction and lactation were not apparent .
	manualset3
129024	1	405371	5	NULL	NULL	0	NULL	stem/progenitor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential of stem/progenitor cells in treating stroke : the missing steps in translating cell therapy from laboratory to clinic .
	manualset3
129025	2	405371	5	NULL	NULL	0	NULL	stroke 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential of stem/progenitor cells in treating stroke : the missing steps in translating cell therapy from laboratory to clinic .
	manualset3
129026	3	405371	5	NULL	NULL	0	NULL	cell therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential of stem/progenitor cells in treating stroke : the missing steps in translating cell therapy from laboratory to clinic .
	manualset3
129027	4	405371	5	NULL	NULL	0	NULL	laboratory 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential of stem/progenitor cells in treating stroke : the missing steps in translating cell therapy from laboratory to clinic .
	manualset3
129028	5	405371	5	NULL	NULL	0	NULL	clinic 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential of stem/progenitor cells in treating stroke : the missing steps in translating cell therapy from laboratory to clinic .
	manualset3
129029	1	405372	5	NULL	NULL	0	NULL	Potential role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential role of SC1 , a cell adhesion molecule , in mammary gland tumors .
	manualset3
129030	2	405372	5	NULL	NULL	0	NULL	SC1, a cell adhesion molecule	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential role of SC1 , a cell adhesion molecule , in mammary gland tumors .
	manualset3
129031	3	405372	5	NULL	NULL	0	NULL	mammary gland tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential role of SC1 , a cell adhesion molecule , in mammary gland tumors .
	manualset3
129032	1	405373	5	NULL	NULL	0	NULL	Potential survival benefits 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential survival benefits of eritoran in severe sepsis patients were associated with high severity of illness .
	manualset3
129033	2	405373	5	NULL	NULL	0	NULL	eritoran 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential survival benefits of eritoran in severe sepsis patients were associated with high severity of illness .
	manualset3
129034	3	405373	5	NULL	NULL	0	NULL	severe sepsis patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential survival benefits of eritoran in severe sepsis patients were associated with high severity of illness .
	manualset3
129035	4	405373	5	NULL	NULL	0	NULL	 high severity of illness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential survival benefits of eritoran in severe sepsis patients were associated with high severity of illness .
	manualset3
129036	1	405374	5	NULL	NULL	0	NULL	Potential vaccinees	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential vaccinees should be queried regarding the diagnosis of atopic dermatitis or eczema in themselves or any member of their household , or regarding the presence of chronic or recurrent rashes consistent with these diagnoses .
	manualset3
129037	2	405374	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential vaccinees should be queried regarding the diagnosis of atopic dermatitis or eczema in themselves or any member of their household , or regarding the presence of chronic or recurrent rashes consistent with these diagnoses .
	manualset3
129038	3	405374	5	NULL	NULL	NULL	NULL	atopic dermatitis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Potential vaccinees should be queried regarding the diagnosis of atopic dermatitis or eczema in themselves or any member of their household , or regarding the presence of chronic or recurrent rashes consistent with these diagnoses .
	manualset3
129039	4	405374	5	NULL	NULL	0	NULL	member 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential vaccinees should be queried regarding the diagnosis of atopic dermatitis or eczema in themselves or any member of their household , or regarding the presence of chronic or recurrent rashes consistent with these diagnoses .
	manualset3
129040	5	405374	5	NULL	NULL	0	NULL	household 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential vaccinees should be queried regarding the diagnosis of atopic dermatitis or eczema in themselves or any member of their household , or regarding the presence of chronic or recurrent rashes consistent with these diagnoses .
	manualset3
129041	6	405374	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential vaccinees should be queried regarding the diagnosis of atopic dermatitis or eczema in themselves or any member of their household , or regarding the presence of chronic or recurrent rashes consistent with these diagnoses .
	manualset3
129042	7	405374	5	NULL	NULL	NULL	NULL	chronic rashes	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Potential vaccinees should be queried regarding the diagnosis of atopic dermatitis or eczema in themselves or any member of their household , or regarding the presence of chronic or recurrent rashes consistent with these diagnoses .
	manualset3
129043	8	405374	5	NULL	NULL	0	NULL	diagnoses 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential vaccinees should be queried regarding the diagnosis of atopic dermatitis or eczema in themselves or any member of their household , or regarding the presence of chronic or recurrent rashes consistent with these diagnoses .
	manualset3
134854	9	405374	5	NULL	NULL	0	NULL	eczema	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential vaccinees should be queried regarding the diagnosis of atopic dermatitis or eczema in themselves or any member of their household , or regarding the presence of chronic or recurrent rashes consistent with these diagnoses .
	manualset3
134855	10	405374	5	NULL	NULL	0	NULL	recurrent rashes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential vaccinees should be queried regarding the diagnosis of atopic dermatitis or eczema in themselves or any member of their household , or regarding the presence of chronic or recurrent rashes consistent with these diagnoses .
	manualset3
129044	1	405375	5	NULL	NULL	0	NULL	antigenic variability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Potentially , antigenic variability exists to the extent that an immune response elicited toward one isolate may not be fully protective against another of the same type .
	manualset3
129045	2	405375	5	NULL	NULL	0	NULL	immune response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Potentially , antigenic variability exists to the extent that an immune response elicited toward one isolate may not be fully protective against another of the same type .
	manualset3
129046	3	405375	5	NULL	NULL	NULL	NULL	one isolate	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Potentially , antigenic variability exists to the extent that an immune response elicited toward one isolate may not be fully protective against another of the same type .
	manualset3
129047	4	405375	5	NULL	NULL	0	NULL	same type	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Potentially , antigenic variability exists to the extent that an immune response elicited toward one isolate may not be fully protective against another of the same type .
	manualset3
129048	1	405376	5	NULL	NULL	0	NULL	lack of evidence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A lack of evidence supporting a role of heritability in the development of idiopathic Parkinson 's disease ( PD ) has implicated exposures to environmental contaminants in the disease etiology .
	manualset3
129049	2	405376	5	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A lack of evidence supporting a role of heritability in the development of idiopathic Parkinson 's disease ( PD ) has implicated exposures to environmental contaminants in the disease etiology .
	manualset3
129050	3	405376	5	NULL	NULL	0	NULL	heritability 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A lack of evidence supporting a role of heritability in the development of idiopathic Parkinson 's disease ( PD ) has implicated exposures to environmental contaminants in the disease etiology .
	manualset3
129051	4	405376	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A lack of evidence supporting a role of heritability in the development of idiopathic Parkinson 's disease ( PD ) has implicated exposures to environmental contaminants in the disease etiology .
	manualset3
129052	5	405376	5	NULL	NULL	0	NULL	Parkinson 's disease ( PD ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A lack of evidence supporting a role of heritability in the development of idiopathic Parkinson 's disease ( PD ) has implicated exposures to environmental contaminants in the disease etiology .
	manualset3
129053	6	405376	5	NULL	NULL	0	NULL	exposures 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A lack of evidence supporting a role of heritability in the development of idiopathic Parkinson 's disease ( PD ) has implicated exposures to environmental contaminants in the disease etiology .
	manualset3
129054	7	405376	5	NULL	NULL	0	NULL	environmental contaminants 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A lack of evidence supporting a role of heritability in the development of idiopathic Parkinson 's disease ( PD ) has implicated exposures to environmental contaminants in the disease etiology .
	manualset3
129055	8	405376	5	NULL	NULL	0	NULL	disease etiology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A lack of evidence supporting a role of heritability in the development of idiopathic Parkinson 's disease ( PD ) has implicated exposures to environmental contaminants in the disease etiology .
	manualset3
129056	1	405377	5	NULL	NULL	0	NULL	monoclonal antibodies 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Potentially , monoclonal antibodies , alone or as carriers of radionuclides , drugs , or toxins , may allow successful diagnosis and treatment of human neuroectodermal tumors .
	manualset3
129057	2	405377	5	NULL	NULL	0	NULL	carriers 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Potentially , monoclonal antibodies , alone or as carriers of radionuclides , drugs , or toxins , may allow successful diagnosis and treatment of human neuroectodermal tumors .
	manualset3
129058	3	405377	5	NULL	NULL	0	NULL	radionuclides 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Potentially , monoclonal antibodies , alone or as carriers of radionuclides , drugs , or toxins , may allow successful diagnosis and treatment of human neuroectodermal tumors .
	manualset3
129059	4	405377	5	NULL	NULL	0	NULL	drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Potentially , monoclonal antibodies , alone or as carriers of radionuclides , drugs , or toxins , may allow successful diagnosis and treatment of human neuroectodermal tumors .
	manualset3
129060	5	405377	5	NULL	NULL	0	NULL	toxins 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Potentially , monoclonal antibodies , alone or as carriers of radionuclides , drugs , or toxins , may allow successful diagnosis and treatment of human neuroectodermal tumors .
	manualset3
129061	6	405377	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Potentially , monoclonal antibodies , alone or as carriers of radionuclides , drugs , or toxins , may allow successful diagnosis and treatment of human neuroectodermal tumors .
	manualset3
129062	7	405377	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Potentially , monoclonal antibodies , alone or as carriers of radionuclides , drugs , or toxins , may allow successful diagnosis and treatment of human neuroectodermal tumors .
	manualset3
129063	8	405377	5	NULL	NULL	NULL	NULL	human neuroectodermal tumors	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Potentially , monoclonal antibodies , alone or as carriers of radionuclides , drugs , or toxins , may allow successful diagnosis and treatment of human neuroectodermal tumors .
	manualset3
129064	1	405378	5	NULL	NULL	0	NULL	Potentiated ATP depletion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Potentiated ATP depletion and pro-apoptotic effects were seen for 3-BrOP combinations with the cytochrome-c-reductase inhibitor antimycin A and the mTOR inhibitor rapamycin .
	manualset3
129065	2	405378	5	NULL	NULL	0	NULL	pro-apoptotic effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Potentiated ATP depletion and pro-apoptotic effects were seen for 3-BrOP combinations with the cytochrome-c-reductase inhibitor antimycin A and the mTOR inhibitor rapamycin .
	manualset3
129066	3	405378	5	NULL	NULL	NULL	NULL	3-BrOP combinations with the cytochrome-c-reductase inhibitor antimycin A	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Potentiated ATP depletion and pro-apoptotic effects were seen for 3-BrOP combinations with the cytochrome-c-reductase inhibitor antimycin A and the mTOR inhibitor rapamycin .
	manualset3
129067	4	405378	5	NULL	NULL	0	NULL	mTOR inhibitor rapamycin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Potentiated ATP depletion and pro-apoptotic effects were seen for 3-BrOP combinations with the cytochrome-c-reductase inhibitor antimycin A and the mTOR inhibitor rapamycin .
	manualset3
129068	1	405379	5	NULL	NULL	0	NULL	Potentiation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Potentiation of CDDP toxicity by PALA was observed when the drug was used in combination with FUra , requiring approximately 6 fold reduction in CDDP dose .
	manualset3
129069	2	405379	5	NULL	NULL	0	NULL	CDDP toxicity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Potentiation of CDDP toxicity by PALA was observed when the drug was used in combination with FUra , requiring approximately 6 fold reduction in CDDP dose .
	manualset3
129070	3	405379	5	NULL	NULL	0	NULL	PALA 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Potentiation of CDDP toxicity by PALA was observed when the drug was used in combination with FUra , requiring approximately 6 fold reduction in CDDP dose .
	manualset3
129071	4	405379	5	NULL	NULL	0	NULL	drug 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Potentiation of CDDP toxicity by PALA was observed when the drug was used in combination with FUra , requiring approximately 6 fold reduction in CDDP dose .
	manualset3
129072	5	405379	5	NULL	NULL	0	NULL	FUra 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Potentiation of CDDP toxicity by PALA was observed when the drug was used in combination with FUra , requiring approximately 6 fold reduction in CDDP dose .
	manualset3
129073	6	405379	5	NULL	NULL	0	NULL	6 fold reduction	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Potentiation of CDDP toxicity by PALA was observed when the drug was used in combination with FUra , requiring approximately 6 fold reduction in CDDP dose .
	manualset3
129074	7	405379	5	NULL	NULL	0	NULL	CDDP dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Potentiation of CDDP toxicity by PALA was observed when the drug was used in combination with FUra , requiring approximately 6 fold reduction in CDDP dose .
	manualset3
129075	1	405380	5	NULL	NULL	0	NULL	Potentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Potentiation of angiotensin II-stimulated vascular contraction by lithium .
	manualset3
129076	2	405380	5	NULL	NULL	0	NULL	 angiotensin II-stimulated vascular contraction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Potentiation of angiotensin II-stimulated vascular contraction by lithium .
	manualset3
129077	3	405380	5	NULL	NULL	0	NULL	lithium 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Potentiation of angiotensin II-stimulated vascular contraction by lithium .
	manualset3
129078	1	405381	5	NULL	NULL	0	NULL	Power optimization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Power optimization of XUV frequency combs for spectroscopy applications ( Invited ) .
	manualset3
129079	2	405381	5	NULL	NULL	0	NULL	XUV frequency combs	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Power optimization of XUV frequency combs for spectroscopy applications ( Invited ) .
	manualset3
129080	3	405381	5	NULL	NULL	0	NULL	spectroscopy applications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Power optimization of XUV frequency combs for spectroscopy applications ( Invited ) .
	manualset3
129081	1	405382	5	NULL	NULL	0	NULL	Power output	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Power output was derived from force-length area or force-time integral calculations , respectively .
	manualset3
129082	2	405382	5	NULL	NULL	0	NULL	force-length area	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Power output was derived from force-length area or force-time integral calculations , respectively .
	manualset3
129083	3	405382	5	NULL	NULL	0	NULL	force-time integral calculations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Power output was derived from force-length area or force-time integral calculations , respectively .
	manualset3
129084	1	405383	5	NULL	NULL	0	NULL	PpPex11p	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PpPex11p transits to peroxisomes via the endoplasmic reticulum ( ER ) .
	manualset3
129085	2	405383	5	NULL	NULL	0	NULL	peroxisomes 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	PpPex11p transits to peroxisomes via the endoplasmic reticulum ( ER ) .
	manualset3
129086	3	405383	5	NULL	NULL	0	NULL	endoplasmic reticulum ( ER )	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	PpPex11p transits to peroxisomes via the endoplasmic reticulum ( ER ) .
	manualset3
129087	1	405384	5	NULL	NULL	0	NULL	Practical Application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Practical Application : This work will be helpful to elucidate the influence of crystallization process and structural properties such as crystal nanostructure and crystal habit on the migration of oil through a crystalline fat matrix .
	manualset3
129088	2	405384	5	NULL	NULL	NULL	NULL	crystallization process	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Practical Application : This work will be helpful to elucidate the influence of crystallization process and structural properties such as crystal nanostructure and crystal habit on the migration of oil through a crystalline fat matrix .
	manualset3
129089	3	405384	5	NULL	NULL	0	NULL	structural properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Practical Application : This work will be helpful to elucidate the influence of crystallization process and structural properties such as crystal nanostructure and crystal habit on the migration of oil through a crystalline fat matrix .
	manualset3
129090	4	405384	5	NULL	NULL	0	NULL	crystal nanostructure 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Practical Application : This work will be helpful to elucidate the influence of crystallization process and structural properties such as crystal nanostructure and crystal habit on the migration of oil through a crystalline fat matrix .
	manualset3
129091	5	405384	5	NULL	NULL	0	NULL	crystal habit	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Practical Application : This work will be helpful to elucidate the influence of crystallization process and structural properties such as crystal nanostructure and crystal habit on the migration of oil through a crystalline fat matrix .
	manualset3
129092	6	405384	5	NULL	NULL	0	NULL	migration 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Practical Application : This work will be helpful to elucidate the influence of crystallization process and structural properties such as crystal nanostructure and crystal habit on the migration of oil through a crystalline fat matrix .
	manualset3
129093	7	405384	5	NULL	NULL	0	NULL	oil 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Practical Application : This work will be helpful to elucidate the influence of crystallization process and structural properties such as crystal nanostructure and crystal habit on the migration of oil through a crystalline fat matrix .
	manualset3
129094	8	405384	5	NULL	NULL	0	NULL	crystalline fat matrix	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Practical Application : This work will be helpful to elucidate the influence of crystallization process and structural properties such as crystal nanostructure and crystal habit on the migration of oil through a crystalline fat matrix .
	manualset3
129096	1	405385	5	NULL	NULL	0	NULL	gastrointestinal and cardiovascular safety concerns	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Practical approaches to minimizing gastrointestinal and cardiovascular safety concerns with COX-2 inhibitors and NSAIDs .
	manualset3
129097	2	405385	5	NULL	NULL	0	NULL	COX-2 inhibitors 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Practical approaches to minimizing gastrointestinal and cardiovascular safety concerns with COX-2 inhibitors and NSAIDs .
	manualset3
129098	3	405385	5	NULL	NULL	0	NULL	NSAIDs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Practical approaches to minimizing gastrointestinal and cardiovascular safety concerns with COX-2 inhibitors and NSAIDs .
	manualset3
129099	1	405386	5	NULL	NULL	0	NULL	dosage regimens	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Practical dosage regimens for streptokinase and urokinase are proposed .
	manualset3
129100	2	405386	5	NULL	NULL	0	NULL	streptokinase 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Practical dosage regimens for streptokinase and urokinase are proposed .
	manualset3
129101	3	405386	5	NULL	NULL	0	NULL	urokinase 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Practical dosage regimens for streptokinase and urokinase are proposed .
	manualset3
129102	1	405387	5	NULL	NULL	0	NULL	Practical significance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Practical significance of the variations ) .
	manualset3
129103	2	405387	5	NULL	NULL	0	NULL	variations 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Practical significance of the variations ) .
	manualset3
129104	1	405388	5	NULL	NULL	0	NULL	Practice plans 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Practice plans of dental school graduating seniors : effects of the Pipeline program .
	manualset3
129105	2	405388	5	NULL	NULL	0	NULL	dental school graduating seniors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Practice plans of dental school graduating seniors : effects of the Pipeline program .
	manualset3
129106	3	405388	5	NULL	NULL	NULL	NULL	Pipeline program 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Practice plans of dental school graduating seniors : effects of the Pipeline program .
	manualset3
129107	1	405389	5	NULL	NULL	0	NULL	Praziquantel 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Praziquantel destroyed mature and developing cercariae within the daughter sporocysts but had no apparent effect on daughter sporocysts ; this may account for the eventual resumption of cercarial production .
	manualset3
129108	2	405389	5	NULL	NULL	0	NULL	mature and developing cercariae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Praziquantel destroyed mature and developing cercariae within the daughter sporocysts but had no apparent effect on daughter sporocysts ; this may account for the eventual resumption of cercarial production .
	manualset3
129109	3	405389	5	NULL	NULL	0	NULL	daughter sporocysts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Praziquantel destroyed mature and developing cercariae within the daughter sporocysts but had no apparent effect on daughter sporocysts ; this may account for the eventual resumption of cercarial production .
	manualset3
129110	4	405389	5	NULL	NULL	0	NULL	daughter sporocysts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Praziquantel destroyed mature and developing cercariae within the daughter sporocysts but had no apparent effect on daughter sporocysts ; this may account for the eventual resumption of cercarial production .
	manualset3
129111	5	405389	5	NULL	NULL	0	NULL	account 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Praziquantel destroyed mature and developing cercariae within the daughter sporocysts but had no apparent effect on daughter sporocysts ; this may account for the eventual resumption of cercarial production .
	manualset3
129112	6	405389	5	NULL	NULL	0	NULL	resumption 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Praziquantel destroyed mature and developing cercariae within the daughter sporocysts but had no apparent effect on daughter sporocysts ; this may account for the eventual resumption of cercarial production .
	manualset3
129113	7	405389	5	NULL	NULL	0	NULL	cercarial production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Praziquantel destroyed mature and developing cercariae within the daughter sporocysts but had no apparent effect on daughter sporocysts ; this may account for the eventual resumption of cercarial production .
	manualset3
129114	1	405390	5	NULL	NULL	0	NULL	Pre-antral hamster	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-antral hamster and human follicles cultured in the presence of follicle stimulating hormone for up to 168 h developed an antral cavity with intact germinal vesicle oocytes .
	manualset3
129115	2	405390	5	NULL	NULL	0	NULL	human follicles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-antral hamster and human follicles cultured in the presence of follicle stimulating hormone for up to 168 h developed an antral cavity with intact germinal vesicle oocytes .
	manualset3
129116	3	405390	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-antral hamster and human follicles cultured in the presence of follicle stimulating hormone for up to 168 h developed an antral cavity with intact germinal vesicle oocytes .
	manualset3
129117	4	405390	5	NULL	NULL	0	NULL	follicle stimulating hormone	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-antral hamster and human follicles cultured in the presence of follicle stimulating hormone for up to 168 h developed an antral cavity with intact germinal vesicle oocytes .
	manualset3
129118	5	405390	5	NULL	NULL	0	NULL	168 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-antral hamster and human follicles cultured in the presence of follicle stimulating hormone for up to 168 h developed an antral cavity with intact germinal vesicle oocytes .
	manualset3
129119	6	405390	5	NULL	NULL	0	NULL	antral cavity	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-antral hamster and human follicles cultured in the presence of follicle stimulating hormone for up to 168 h developed an antral cavity with intact germinal vesicle oocytes .
	manualset3
129120	7	405390	5	NULL	NULL	0	NULL	intact germinal vesicle oocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-antral hamster and human follicles cultured in the presence of follicle stimulating hormone for up to 168 h developed an antral cavity with intact germinal vesicle oocytes .
	manualset3
129121	1	405391	5	NULL	NULL	0	NULL	Pre-incubation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-incubation with glutamate also increased the net uptake of non-radioactive glutamate , providing evidence that the increase in accumulation of L - ( ( 3 ) H ) - glutamate was not related to an increase in intracellular glutamate and a subsequent increase in exchange of intracellular non-radioactive glutamate for extracellular radioactive glutamate .
	manualset3
129122	2	405391	5	NULL	NULL	0	NULL	glutamate 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-incubation with glutamate also increased the net uptake of non-radioactive glutamate , providing evidence that the increase in accumulation of L - ( ( 3 ) H ) - glutamate was not related to an increase in intracellular glutamate and a subsequent increase in exchange of intracellular non-radioactive glutamate for extracellular radioactive glutamate .
	manualset3
129123	3	405391	5	NULL	NULL	0	NULL	net uptake	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-incubation with glutamate also increased the net uptake of non-radioactive glutamate , providing evidence that the increase in accumulation of L - ( ( 3 ) H ) - glutamate was not related to an increase in intracellular glutamate and a subsequent increase in exchange of intracellular non-radioactive glutamate for extracellular radioactive glutamate .
	manualset3
129124	4	405391	5	NULL	NULL	0	NULL	non-radioactive glutamate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-incubation with glutamate also increased the net uptake of non-radioactive glutamate , providing evidence that the increase in accumulation of L - ( ( 3 ) H ) - glutamate was not related to an increase in intracellular glutamate and a subsequent increase in exchange of intracellular non-radioactive glutamate for extracellular radioactive glutamate .
	manualset3
129125	5	405391	5	NULL	NULL	0	NULL	evidence 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-incubation with glutamate also increased the net uptake of non-radioactive glutamate , providing evidence that the increase in accumulation of L - ( ( 3 ) H ) - glutamate was not related to an increase in intracellular glutamate and a subsequent increase in exchange of intracellular non-radioactive glutamate for extracellular radioactive glutamate .
	manualset3
129126	6	405391	5	NULL	NULL	0	NULL	accumulation 	p												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-incubation with glutamate also increased the net uptake of non-radioactive glutamate , providing evidence that the increase in accumulation of L - ( ( 3 ) H ) - glutamate was not related to an increase in intracellular glutamate and a subsequent increase in exchange of intracellular non-radioactive glutamate for extracellular radioactive glutamate .
	manualset3
129127	7	405391	5	NULL	NULL	0	NULL	L - ( ( 3 ) H ) - glutamate	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-incubation with glutamate also increased the net uptake of non-radioactive glutamate , providing evidence that the increase in accumulation of L - ( ( 3 ) H ) - glutamate was not related to an increase in intracellular glutamate and a subsequent increase in exchange of intracellular non-radioactive glutamate for extracellular radioactive glutamate .
	manualset3
129128	8	405391	5	NULL	NULL	0	NULL	intracellular glutamate	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-incubation with glutamate also increased the net uptake of non-radioactive glutamate , providing evidence that the increase in accumulation of L - ( ( 3 ) H ) - glutamate was not related to an increase in intracellular glutamate and a subsequent increase in exchange of intracellular non-radioactive glutamate for extracellular radioactive glutamate .
	manualset3
129129	9	405391	5	NULL	NULL	NULL	NULL	exchange 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pre-incubation with glutamate also increased the net uptake of non-radioactive glutamate , providing evidence that the increase in accumulation of L - ( ( 3 ) H ) - glutamate was not related to an increase in intracellular glutamate and a subsequent increase in exchange of intracellular non-radioactive glutamate for extracellular radioactive glutamate .
	manualset3
129130	10	405391	5	NULL	NULL	0	NULL	intracellular non-radioactive glutamate 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-incubation with glutamate also increased the net uptake of non-radioactive glutamate , providing evidence that the increase in accumulation of L - ( ( 3 ) H ) - glutamate was not related to an increase in intracellular glutamate and a subsequent increase in exchange of intracellular non-radioactive glutamate for extracellular radioactive glutamate .
	manualset3
129131	11	405391	5	NULL	NULL	0	NULL	extracellular radioactive glutamate	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-incubation with glutamate also increased the net uptake of non-radioactive glutamate , providing evidence that the increase in accumulation of L - ( ( 3 ) H ) - glutamate was not related to an increase in intracellular glutamate and a subsequent increase in exchange of intracellular non-radioactive glutamate for extracellular radioactive glutamate .
	manualset3
129132	1	405392	5	NULL	NULL	0	NULL	large aquatic herb , Nelumbo nucifera Gaertn	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A large aquatic herb , Nelumbo nucifera Gaertn , has psychopharmacological effects similar to minor tranquillizers and antistress agents .
	manualset3
129133	2	405392	5	NULL	NULL	0	NULL	psychopharmacological effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A large aquatic herb , Nelumbo nucifera Gaertn , has psychopharmacological effects similar to minor tranquillizers and antistress agents .
	manualset3
129134	3	405392	5	NULL	NULL	NULL	NULL	minor tranquillizers	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A large aquatic herb , Nelumbo nucifera Gaertn , has psychopharmacological effects similar to minor tranquillizers and antistress agents .
	manualset3
129135	4	405392	5	NULL	NULL	0	NULL	antistress agents	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A large aquatic herb , Nelumbo nucifera Gaertn , has psychopharmacological effects similar to minor tranquillizers and antistress agents .
	manualset3
129136	1	405393	5	NULL	NULL	NULL	NULL	Pre-meal human regular insulin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pre-meal human regular insulin was used with ultralente insulins and comprised 39 + / - 2 % of the total daily insulin dose .
	manualset3
129137	2	405393	5	NULL	NULL	NULL	NULL	ultralente insulins	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pre-meal human regular insulin was used with ultralente insulins and comprised 39 + / - 2 % of the total daily insulin dose .
	manualset3
129138	3	405393	5	NULL	NULL	0	NULL	39 + / - 2 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-meal human regular insulin was used with ultralente insulins and comprised 39 + / - 2 % of the total daily insulin dose .
	manualset3
129139	4	405393	5	NULL	NULL	0	NULL	total daily insulin dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-meal human regular insulin was used with ultralente insulins and comprised 39 + / - 2 % of the total daily insulin dose .
	manualset3
129140	1	405394	5	NULL	NULL	0	NULL	Pre-operational viral replication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-operational viral replication , immunosuppression degree , and disease types play an important role in hepatitis B recurrence .
	manualset3
129141	2	405394	5	NULL	NULL	0	NULL	immunosuppression degree	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-operational viral replication , immunosuppression degree , and disease types play an important role in hepatitis B recurrence .
	manualset3
129142	3	405394	5	NULL	NULL	0	NULL	disease types	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-operational viral replication , immunosuppression degree , and disease types play an important role in hepatitis B recurrence .
	manualset3
129143	4	405394	5	NULL	NULL	0	NULL	important role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-operational viral replication , immunosuppression degree , and disease types play an important role in hepatitis B recurrence .
	manualset3
129144	5	405394	5	NULL	NULL	0	NULL	hepatitis B recurrence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-operational viral replication , immunosuppression degree , and disease types play an important role in hepatitis B recurrence .
	manualset3
129145	1	405395	5	NULL	NULL	0	NULL	Pre-operative predeposit autologous donation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-operative predeposit autologous donation in children presenting for elective surgery : a review .
	manualset3
129146	2	405395	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-operative predeposit autologous donation in children presenting for elective surgery : a review .
	manualset3
129147	3	405395	5	NULL	NULL	0	NULL	elective surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-operative predeposit autologous donation in children presenting for elective surgery : a review .
	manualset3
129148	4	405395	5	NULL	NULL	0	NULL	review 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-operative predeposit autologous donation in children presenting for elective surgery : a review .
	manualset3
129149	1	405396	5	NULL	NULL	0	NULL	BP 157 + / -16 / 88 + / -10 mm Hg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-switching BP 157 + / -16 / 88 + / -10 mm Hg promptly decreased and maintained a steady state , reaching 132 + / -15 / 77 + / -9 mm Hg ( P & lt ; 0.001 ) 1 year later .
	manualset3
129150	2	405396	5	NULL	NULL	0	NULL	steady state	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-switching BP 157 + / -16 / 88 + / -10 mm Hg promptly decreased and maintained a steady state , reaching 132 + / -15 / 77 + / -9 mm Hg ( P & lt ; 0.001 ) 1 year later .
	manualset3
129151	3	405396	5	NULL	NULL	0	NULL	132 + / -15 / 77 + / -9 mm Hg ( P & lt ; 0.001 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-switching BP 157 + / -16 / 88 + / -10 mm Hg promptly decreased and maintained a steady state , reaching 132 + / -15 / 77 + / -9 mm Hg ( P & lt ; 0.001 ) 1 year later .
	manualset3
129152	4	405396	5	NULL	NULL	0	NULL	1 year	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-switching BP 157 + / -16 / 88 + / -10 mm Hg promptly decreased and maintained a steady state , reaching 132 + / -15 / 77 + / -9 mm Hg ( P & lt ; 0.001 ) 1 year later .
	manualset3
129153	1	405397	5	NULL	NULL	0	NULL	Pre - and postoperative evaluation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre - and postoperative evaluation included the Lysholm knee function scoring scale , Tegner activity rating scale and KT-1000 arthrometer measurements .
	manualset3
129154	2	405397	5	NULL	NULL	0	NULL	Lysholm knee function scoring scale 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre - and postoperative evaluation included the Lysholm knee function scoring scale , Tegner activity rating scale and KT-1000 arthrometer measurements .
	manualset3
129155	3	405397	5	NULL	NULL	NULL	NULL	Tegner activity rating scale	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pre - and postoperative evaluation included the Lysholm knee function scoring scale , Tegner activity rating scale and KT-1000 arthrometer measurements .
	manualset3
129156	4	405397	5	NULL	NULL	0	NULL	KT-1000 arthrometer measurements	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre - and postoperative evaluation included the Lysholm knee function scoring scale , Tegner activity rating scale and KT-1000 arthrometer measurements .
	manualset3
129157	1	405398	5	NULL	NULL	0	NULL	Pre - and postsynaptic receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre - and postsynaptic receptors in catecholaminergic transmission .
	manualset3
129158	2	405398	5	NULL	NULL	0	NULL	catecholaminergic transmission	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre - and postsynaptic receptors in catecholaminergic transmission .
	manualset3
129159	1	405399	5	NULL	NULL	0	NULL	Preassembly 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Preassembly of membrane-active peptides is an important factor in their selectivity toward target cells .
	manualset3
129160	2	405399	5	NULL	NULL	0	NULL	membrane-active peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Preassembly of membrane-active peptides is an important factor in their selectivity toward target cells .
	manualset3
129161	3	405399	5	NULL	NULL	0	NULL	important factor 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preassembly of membrane-active peptides is an important factor in their selectivity toward target cells .
	manualset3
129162	4	405399	5	NULL	NULL	0	NULL	selectivity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Preassembly of membrane-active peptides is an important factor in their selectivity toward target cells .
	manualset3
129163	5	405399	5	NULL	NULL	0	NULL	target cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Preassembly of membrane-active peptides is an important factor in their selectivity toward target cells .
	manualset3
129164	1	405400	5	NULL	NULL	NULL	NULL	 large body	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A large body of cytogenetic data indicates that most TS features are due to reduced dosage of genes on the short arm of the X chromosome ( Xp ) .
	manualset3
129165	2	405400	5	NULL	NULL	0	NULL	cytogenetic data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A large body of cytogenetic data indicates that most TS features are due to reduced dosage of genes on the short arm of the X chromosome ( Xp ) .
	manualset3
129166	3	405400	5	NULL	NULL	0	NULL	TS features 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A large body of cytogenetic data indicates that most TS features are due to reduced dosage of genes on the short arm of the X chromosome ( Xp ) .
	manualset3
129167	4	405400	5	NULL	NULL	0	NULL	reduced dosage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A large body of cytogenetic data indicates that most TS features are due to reduced dosage of genes on the short arm of the X chromosome ( Xp ) .
	manualset3
129168	5	405400	5	NULL	NULL	0	NULL	genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A large body of cytogenetic data indicates that most TS features are due to reduced dosage of genes on the short arm of the X chromosome ( Xp ) .
	manualset3
129169	6	405400	5	NULL	NULL	0	NULL	short arm of the X chromosome ( Xp ) 	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	A large body of cytogenetic data indicates that most TS features are due to reduced dosage of genes on the short arm of the X chromosome ( Xp ) .
	manualset3
129170	1	405401	5	NULL	NULL	0	NULL	Prebranchial injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prebranchial injection of adenosine or the A1-receptor agonist N6-cyclopentyl-adenosine ( CPA ) constricted the distal portion of the filament vasculature , which coincided with an increase of PVA .
	manualset3
129171	2	405401	5	NULL	NULL	0	NULL	adenosine	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Prebranchial injection of adenosine or the A1-receptor agonist N6-cyclopentyl-adenosine ( CPA ) constricted the distal portion of the filament vasculature , which coincided with an increase of PVA .
	manualset3
129172	3	405401	5	NULL	NULL	0	NULL	A1-receptor agonist N6-cyclopentyl-adenosine ( CPA )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Prebranchial injection of adenosine or the A1-receptor agonist N6-cyclopentyl-adenosine ( CPA ) constricted the distal portion of the filament vasculature , which coincided with an increase of PVA .
	manualset3
129173	4	405401	5	NULL	NULL	0	NULL	distal portion of the filament vasculature	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Prebranchial injection of adenosine or the A1-receptor agonist N6-cyclopentyl-adenosine ( CPA ) constricted the distal portion of the filament vasculature , which coincided with an increase of PVA .
	manualset3
129174	5	405401	5	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prebranchial injection of adenosine or the A1-receptor agonist N6-cyclopentyl-adenosine ( CPA ) constricted the distal portion of the filament vasculature , which coincided with an increase of PVA .
	manualset3
129175	6	405401	5	NULL	NULL	0	NULL	PVA	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Prebranchial injection of adenosine or the A1-receptor agonist N6-cyclopentyl-adenosine ( CPA ) constricted the distal portion of the filament vasculature , which coincided with an increase of PVA .
	manualset3
129176	1	405402	5	NULL	NULL	0	NULL	Precipitation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Precipitation of Y89-5-3 was similar to that of very flocculent yeast ( 80 % ) at 75.95 % .
	manualset3
129177	2	405402	5	NULL	NULL	0	NULL	Y89-5-3	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Precipitation of Y89-5-3 was similar to that of very flocculent yeast ( 80 % ) at 75.95 % .
	manualset3
129178	3	405402	5	NULL	NULL	0	NULL	flocculent yeast 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Precipitation of Y89-5-3 was similar to that of very flocculent yeast ( 80 % ) at 75.95 % .
	manualset3
129179	4	405402	5	NULL	NULL	0	NULL	 80 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Precipitation of Y89-5-3 was similar to that of very flocculent yeast ( 80 % ) at 75.95 % .
	manualset3
129180	5	405402	5	NULL	NULL	0	NULL	75.95 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Precipitation of Y89-5-3 was similar to that of very flocculent yeast ( 80 % ) at 75.95 % .
	manualset3
129181	1	405403	5	NULL	NULL	0	NULL	Preclinical Alzheimer disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Preclinical Alzheimer disease : neuropsychological test performance 1.5 to 8 years prior to onset .
	manualset3
129182	2	405403	5	NULL	NULL	NULL	NULL	neuropsychological test performance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Preclinical Alzheimer disease : neuropsychological test performance 1.5 to 8 years prior to onset .
	manualset3
129183	3	405403	5	NULL	NULL	0	NULL	1.5 to 8 years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Preclinical Alzheimer disease : neuropsychological test performance 1.5 to 8 years prior to onset .
	manualset3
129184	4	405403	5	NULL	NULL	0	NULL	onset	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Preclinical Alzheimer disease : neuropsychological test performance 1.5 to 8 years prior to onset .
	manualset3
129185	1	405404	5	NULL	NULL	0	NULL	Precontraction brachial arterial blood flow	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Precontraction brachial arterial blood flow ( Doppler ultrasound ) was reduced with EC100 or EC160 ( 56 % and 39 % of baseline value , respectively ) compared with no external compression ( control ) .
	manualset3
129186	2	405404	5	NULL	NULL	0	NULL	Doppler ultrasound	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Precontraction brachial arterial blood flow ( Doppler ultrasound ) was reduced with EC100 or EC160 ( 56 % and 39 % of baseline value , respectively ) compared with no external compression ( control ) .
	manualset3
129187	3	405404	5	NULL	NULL	0	NULL	EC100 or EC160	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Precontraction brachial arterial blood flow ( Doppler ultrasound ) was reduced with EC100 or EC160 ( 56 % and 39 % of baseline value , respectively ) compared with no external compression ( control ) .
	manualset3
129188	4	405404	5	NULL	NULL	0	NULL	56 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Precontraction brachial arterial blood flow ( Doppler ultrasound ) was reduced with EC100 or EC160 ( 56 % and 39 % of baseline value , respectively ) compared with no external compression ( control ) .
	manualset3
129189	5	405404	5	NULL	NULL	0	NULL	39 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Precontraction brachial arterial blood flow ( Doppler ultrasound ) was reduced with EC100 or EC160 ( 56 % and 39 % of baseline value , respectively ) compared with no external compression ( control ) .
	manualset3
129190	6	405404	5	NULL	NULL	0	NULL	baseline value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Precontraction brachial arterial blood flow ( Doppler ultrasound ) was reduced with EC100 or EC160 ( 56 % and 39 % of baseline value , respectively ) compared with no external compression ( control ) .
	manualset3
129191	7	405404	5	NULL	NULL	0	NULL	external compression	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Precontraction brachial arterial blood flow ( Doppler ultrasound ) was reduced with EC100 or EC160 ( 56 % and 39 % of baseline value , respectively ) compared with no external compression ( control ) .
	manualset3
129192	8	405404	5	NULL	NULL	0	NULL	control	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Precontraction brachial arterial blood flow ( Doppler ultrasound ) was reduced with EC100 or EC160 ( 56 % and 39 % of baseline value , respectively ) compared with no external compression ( control ) .
	manualset3
129193	1	405405	5	NULL	NULL	0	NULL	Precursor lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Precursor lesions including ductal hyperplasia and hyperplastic alveolar nodules were present by the age of 4 months .
	manualset3
129194	2	405405	5	NULL	NULL	0	NULL	ductal hyperplasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Precursor lesions including ductal hyperplasia and hyperplastic alveolar nodules were present by the age of 4 months .
	manualset3
129195	3	405405	5	NULL	NULL	0	NULL	hyperplastic alveolar nodules	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Precursor lesions including ductal hyperplasia and hyperplastic alveolar nodules were present by the age of 4 months .
	manualset3
129196	4	405405	5	NULL	NULL	0	NULL	age	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Precursor lesions including ductal hyperplasia and hyperplastic alveolar nodules were present by the age of 4 months .
	manualset3
129197	5	405405	5	NULL	NULL	0	NULL	4 months	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Precursor lesions including ductal hyperplasia and hyperplastic alveolar nodules were present by the age of 4 months .
	manualset3
129198	1	405406	5	NULL	NULL	NULL	NULL	Predator stress	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Predator stress is a traumatic experience inducing long-lasting fear , but not in all rodents .
	manualset3
129199	2	405406	5	NULL	NULL	NULL	NULL	traumatic experience	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Predator stress is a traumatic experience inducing long-lasting fear , but not in all rodents .
	manualset3
129200	3	405406	5	NULL	NULL	0	NULL	long-lasting fear	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Predator stress is a traumatic experience inducing long-lasting fear , but not in all rodents .
	manualset3
129201	4	405406	5	NULL	NULL	0	NULL	rodents	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Predator stress is a traumatic experience inducing long-lasting fear , but not in all rodents .
	manualset3
129202	1	405407	5	NULL	NULL	0	NULL	Predicted deficits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Predicted deficits were seen on trailmaking ( relatives of ADHD combined type only ) , stop-signal reaction times ( relatives of girls only ) , and response variability ( mothers only ) but not on naming or output speed .
	manualset3
129203	2	405407	5	NULL	NULL	0	NULL	trailmaking	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Predicted deficits were seen on trailmaking ( relatives of ADHD combined type only ) , stop-signal reaction times ( relatives of girls only ) , and response variability ( mothers only ) but not on naming or output speed .
	manualset3
129204	3	405407	5	NULL	NULL	0	NULL	relatives	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Predicted deficits were seen on trailmaking ( relatives of ADHD combined type only ) , stop-signal reaction times ( relatives of girls only ) , and response variability ( mothers only ) but not on naming or output speed .
	manualset3
129205	4	405407	5	NULL	NULL	NULL	NULL	ADHD combined type	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Predicted deficits were seen on trailmaking ( relatives of ADHD combined type only ) , stop-signal reaction times ( relatives of girls only ) , and response variability ( mothers only ) but not on naming or output speed .
	manualset3
129206	5	405407	5	NULL	NULL	NULL	NULL	stop-signal reaction times	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Predicted deficits were seen on trailmaking ( relatives of ADHD combined type only ) , stop-signal reaction times ( relatives of girls only ) , and response variability ( mothers only ) but not on naming or output speed .
	manualset3
129207	6	405407	5	NULL	NULL	0	NULL	relatives	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Predicted deficits were seen on trailmaking ( relatives of ADHD combined type only ) , stop-signal reaction times ( relatives of girls only ) , and response variability ( mothers only ) but not on naming or output speed .
	manualset3
129208	7	405407	5	NULL	NULL	0	NULL	girls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Predicted deficits were seen on trailmaking ( relatives of ADHD combined type only ) , stop-signal reaction times ( relatives of girls only ) , and response variability ( mothers only ) but not on naming or output speed .
	manualset3
129209	8	405407	5	NULL	NULL	0	NULL	response variability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Predicted deficits were seen on trailmaking ( relatives of ADHD combined type only ) , stop-signal reaction times ( relatives of girls only ) , and response variability ( mothers only ) but not on naming or output speed .
	manualset3
129210	9	405407	5	NULL	NULL	0	NULL	mothers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Predicted deficits were seen on trailmaking ( relatives of ADHD combined type only ) , stop-signal reaction times ( relatives of girls only ) , and response variability ( mothers only ) but not on naming or output speed .
	manualset3
129211	10	405407	5	NULL	NULL	0	NULL	naming	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Predicted deficits were seen on trailmaking ( relatives of ADHD combined type only ) , stop-signal reaction times ( relatives of girls only ) , and response variability ( mothers only ) but not on naming or output speed .
	manualset3
129212	11	405407	5	NULL	NULL	0	NULL	output speed	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Predicted deficits were seen on trailmaking ( relatives of ADHD combined type only ) , stop-signal reaction times ( relatives of girls only ) , and response variability ( mothers only ) but not on naming or output speed .
	manualset3
129213	1	405408	5	NULL	NULL	0	NULL	carcinogenicity	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Predicting carcinogenicity with short-term tests : biological models and operational approaches .
	manualset3
129214	2	405408	5	NULL	NULL	0	NULL	short-term tests	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Predicting carcinogenicity with short-term tests : biological models and operational approaches .
	manualset3
129215	3	405408	5	NULL	NULL	0	NULL	biological models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Predicting carcinogenicity with short-term tests : biological models and operational approaches .
	manualset3
129216	4	405408	5	NULL	NULL	0	NULL	operational approaches	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Predicting carcinogenicity with short-term tests : biological models and operational approaches .
	manualset3
129217	1	405409	5	NULL	NULL	0	NULL	deep venous thrombosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Predicting deep venous thrombosis in pregnancy : out in `` LEFt '' field ?
	manualset3
129218	2	405409	5	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Predicting deep venous thrombosis in pregnancy : out in `` LEFt '' field ?
	manualset3
129219	1	405410	5	NULL	NULL	0	NULL	evidence	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A large body of evidence indicates that ligand-gated channels may open spontaneously , exhibiting a basal activity in the absence of the neurotransmitter .
	manualset3
129220	2	405410	5	NULL	NULL	0	NULL	ligand-gated channels 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A large body of evidence indicates that ligand-gated channels may open spontaneously , exhibiting a basal activity in the absence of the neurotransmitter .
	manualset3
129221	3	405410	5	NULL	NULL	0	NULL	basal activity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A large body of evidence indicates that ligand-gated channels may open spontaneously , exhibiting a basal activity in the absence of the neurotransmitter .
	manualset3
129222	4	405410	5	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A large body of evidence indicates that ligand-gated channels may open spontaneously , exhibiting a basal activity in the absence of the neurotransmitter .
	manualset3
129223	5	405410	5	NULL	NULL	0	NULL	neurotransmitter	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A large body of evidence indicates that ligand-gated channels may open spontaneously , exhibiting a basal activity in the absence of the neurotransmitter .
	manualset3
134856	6	405410	5	NULL	NULL	0	NULL	large body	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A large body of evidence indicates that ligand-gated channels may open spontaneously , exhibiting a basal activity in the absence of the neurotransmitter .
	manualset3
129224	1	405411	5	NULL	NULL	0	NULL	viability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Predicting overall viability of cord blood harvests .
	manualset3
129225	2	405411	5	NULL	NULL	0	NULL	cord blood harvests	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Predicting overall viability of cord blood harvests .
	manualset3
129226	1	405412	5	NULL	NULL	0	NULL	Prediction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prediction of cardiovascular complications in patients with prostatic cancer treated with estrogen .
	manualset3
129227	2	405412	5	NULL	NULL	0	NULL	cardiovascular complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prediction of cardiovascular complications in patients with prostatic cancer treated with estrogen .
	manualset3
129228	3	405412	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Prediction of cardiovascular complications in patients with prostatic cancer treated with estrogen .
	manualset3
129229	4	405412	5	NULL	NULL	0	NULL	prostatic cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Prediction of cardiovascular complications in patients with prostatic cancer treated with estrogen .
	manualset3
129230	5	405412	5	NULL	NULL	0	NULL	estrogen	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Prediction of cardiovascular complications in patients with prostatic cancer treated with estrogen .
	manualset3
129231	1	405413	5	NULL	NULL	0	NULL	Prediction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prediction of long-term complications associated with aortic valve prostheses .
	manualset3
129232	2	405413	5	NULL	NULL	0	NULL	long-term complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prediction of long-term complications associated with aortic valve prostheses .
	manualset3
129233	3	405413	5	NULL	NULL	0	NULL	aortic valve prostheses	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Prediction of long-term complications associated with aortic valve prostheses .
	manualset3
129234	1	405414	5	NULL	NULL	0	NULL	Prediction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prediction of reflex sympathetic dystrophy in hemiplegic patients by electromyographic study .
	manualset3
129235	2	405414	5	NULL	NULL	0	NULL	reflex sympathetic dystrophy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Prediction of reflex sympathetic dystrophy in hemiplegic patients by electromyographic study .
	manualset3
129236	3	405414	5	NULL	NULL	0	NULL	hemiplegic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Prediction of reflex sympathetic dystrophy in hemiplegic patients by electromyographic study .
	manualset3
129237	4	405414	5	NULL	NULL	0	NULL	electromyographic study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Prediction of reflex sympathetic dystrophy in hemiplegic patients by electromyographic study .
	manualset3
129292	1	405415	5	NULL	NULL	0	NULL	Predictions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictions from questionnaire information for high ETS exposure were not always the same as those indicated by urinary cotinine emphasizing that the bioindicator , which indicates the actual inhalation of ETS , is a better predictor of exposure than responses from a questionnaire .
	manualset3
129293	2	405415	5	NULL	NULL	0	NULL	questionnaire information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictions from questionnaire information for high ETS exposure were not always the same as those indicated by urinary cotinine emphasizing that the bioindicator , which indicates the actual inhalation of ETS , is a better predictor of exposure than responses from a questionnaire .
	manualset3
129294	3	405415	5	NULL	NULL	NULL	NULL	high ETS exposure	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Predictions from questionnaire information for high ETS exposure were not always the same as those indicated by urinary cotinine emphasizing that the bioindicator , which indicates the actual inhalation of ETS , is a better predictor of exposure than responses from a questionnaire .
	manualset3
129295	4	405415	5	NULL	NULL	0	NULL	urinary cotinine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictions from questionnaire information for high ETS exposure were not always the same as those indicated by urinary cotinine emphasizing that the bioindicator , which indicates the actual inhalation of ETS , is a better predictor of exposure than responses from a questionnaire .
	manualset3
129296	5	405415	5	NULL	NULL	0	NULL	bioindicator	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictions from questionnaire information for high ETS exposure were not always the same as those indicated by urinary cotinine emphasizing that the bioindicator , which indicates the actual inhalation of ETS , is a better predictor of exposure than responses from a questionnaire .
	manualset3
129297	6	405415	5	NULL	NULL	0	NULL	inhalation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictions from questionnaire information for high ETS exposure were not always the same as those indicated by urinary cotinine emphasizing that the bioindicator , which indicates the actual inhalation of ETS , is a better predictor of exposure than responses from a questionnaire .
	manualset3
129298	7	405415	5	NULL	NULL	0	NULL	ETS	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictions from questionnaire information for high ETS exposure were not always the same as those indicated by urinary cotinine emphasizing that the bioindicator , which indicates the actual inhalation of ETS , is a better predictor of exposure than responses from a questionnaire .
	manualset3
129299	8	405415	5	NULL	NULL	0	NULL	predictor	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictions from questionnaire information for high ETS exposure were not always the same as those indicated by urinary cotinine emphasizing that the bioindicator , which indicates the actual inhalation of ETS , is a better predictor of exposure than responses from a questionnaire .
	manualset3
129300	9	405415	5	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictions from questionnaire information for high ETS exposure were not always the same as those indicated by urinary cotinine emphasizing that the bioindicator , which indicates the actual inhalation of ETS , is a better predictor of exposure than responses from a questionnaire .
	manualset3
129301	10	405415	5	NULL	NULL	0	NULL	responses	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictions from questionnaire information for high ETS exposure were not always the same as those indicated by urinary cotinine emphasizing that the bioindicator , which indicates the actual inhalation of ETS , is a better predictor of exposure than responses from a questionnaire .
	manualset3
129302	11	405415	5	NULL	NULL	0	NULL	questionnaire	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictions from questionnaire information for high ETS exposure were not always the same as those indicated by urinary cotinine emphasizing that the bioindicator , which indicates the actual inhalation of ETS , is a better predictor of exposure than responses from a questionnaire .
	manualset3
129303	1	405416	5	NULL	NULL	0	NULL	Predictive factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictive factors of ventricular fibrillation triggered by pause-dependent torsades de pointes associated with acquired long QT interval : role of QT dispersion and left ventricular function .
	manualset3
129304	2	405416	5	NULL	NULL	0	NULL	ventricular fibrillation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictive factors of ventricular fibrillation triggered by pause-dependent torsades de pointes associated with acquired long QT interval : role of QT dispersion and left ventricular function .
	manualset3
129305	3	405416	5	NULL	NULL	0	NULL	torsades de pointes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictive factors of ventricular fibrillation triggered by pause-dependent torsades de pointes associated with acquired long QT interval : role of QT dispersion and left ventricular function .
	manualset3
129306	4	405416	5	NULL	NULL	0	NULL	acquired long QT interval	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictive factors of ventricular fibrillation triggered by pause-dependent torsades de pointes associated with acquired long QT interval : role of QT dispersion and left ventricular function .
	manualset3
129307	5	405416	5	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictive factors of ventricular fibrillation triggered by pause-dependent torsades de pointes associated with acquired long QT interval : role of QT dispersion and left ventricular function .
	manualset3
129308	6	405416	5	NULL	NULL	0	NULL	QT dispersion	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictive factors of ventricular fibrillation triggered by pause-dependent torsades de pointes associated with acquired long QT interval : role of QT dispersion and left ventricular function .
	manualset3
129471	7	405416	5	NULL	NULL	NULL	NULL	left ventricular function	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Predictive factors of ventricular fibrillation triggered by pause-dependent torsades de pointes associated with acquired long QT interval : role of QT dispersion and left ventricular function .
	manualset3
129472	1	405417	5	NULL	NULL	0	NULL	Predictive performance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictive performance of renal function equations for patients with chronic kidney disease and normal serum creatinine levels .
	manualset3
129473	2	405417	5	NULL	NULL	0	NULL	renal function equations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictive performance of renal function equations for patients with chronic kidney disease and normal serum creatinine levels .
	manualset3
130012	3	405417	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictive performance of renal function equations for patients with chronic kidney disease and normal serum creatinine levels .
	manualset3
130013	4	405417	5	NULL	NULL	0	NULL	chronic kidney disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictive performance of renal function equations for patients with chronic kidney disease and normal serum creatinine levels .
	manualset3
130014	5	405417	5	NULL	NULL	0	NULL	normal serum creatinine levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictive performance of renal function equations for patients with chronic kidney disease and normal serum creatinine levels .
	manualset3
130015	1	405418	5	NULL	NULL	0	NULL	Predictive regression equations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictive regression equations and clinical uses of peripheral pulse timing characteristics in children .
	manualset3
130016	2	405418	5	NULL	NULL	0	NULL	peripheral pulse timing characteristics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictive regression equations and clinical uses of peripheral pulse timing characteristics in children .
	manualset3
130017	3	405418	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictive regression equations and clinical uses of peripheral pulse timing characteristics in children .
	manualset3
134857	4	405418	5	NULL	NULL	0	NULL	clinical uses	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictive regression equations and clinical uses of peripheral pulse timing characteristics in children .
	manualset3
130018	1	405419	5	NULL	NULL	0	NULL	Predictors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictors included mean daily AT , season , day of week and public holidays for the base model .
	manualset3
130019	2	405419	5	NULL	NULL	0	NULL	mean daily AT	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictors included mean daily AT , season , day of week and public holidays for the base model .
	manualset3
130020	3	405419	5	NULL	NULL	0	NULL	season 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictors included mean daily AT , season , day of week and public holidays for the base model .
	manualset3
130021	4	405419	5	NULL	NULL	0	NULL	day of week	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictors included mean daily AT , season , day of week and public holidays for the base model .
	manualset3
130022	5	405419	5	NULL	NULL	0	NULL	public holidays	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictors included mean daily AT , season , day of week and public holidays for the base model .
	manualset3
130023	6	405419	5	NULL	NULL	0	NULL	base model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictors included mean daily AT , season , day of week and public holidays for the base model .
	manualset3
130024	1	405420	5	NULL	NULL	0	NULL	Predictors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictors of late death in 5-year survivors of heart transplantation .
	manualset3
130025	2	405420	5	NULL	NULL	0	NULL	late death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictors of late death in 5-year survivors of heart transplantation .
	manualset3
130026	3	405420	5	NULL	NULL	0	NULL	5-year survivors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictors of late death in 5-year survivors of heart transplantation .
	manualset3
130027	4	405420	5	NULL	NULL	0	NULL	heart transplantation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictors of late death in 5-year survivors of heart transplantation .
	manualset3
130028	1	405421	5	NULL	NULL	0	NULL	Predictors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictors of service use are reported and contrasted with previous findings .
	manualset3
130029	2	405421	5	NULL	NULL	0	NULL	previous findings	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictors of service use are reported and contrasted with previous findings .
	manualset3
134858	3	405421	5	NULL	NULL	0	NULL	service use	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictors of service use are reported and contrasted with previous findings .
	manualset3
130030	1	405422	5	NULL	NULL	0	NULL	Predictors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictors of success in an obesity-control program are discussed .
	manualset3
130031	2	405422	5	NULL	NULL	0	NULL	success 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictors of success in an obesity-control program are discussed .
	manualset3
130032	3	405422	5	NULL	NULL	0	NULL	obesity-control program	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictors of success in an obesity-control program are discussed .
	manualset3
130033	1	405423	5	NULL	NULL	0	NULL	Predisposing factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Predisposing factors were chronic alcoholism ( osteonecrosis ) and septicemia due to intravenous drug abuse ( suppurative arthritis ) .
	manualset3
130034	2	405423	5	NULL	NULL	0	NULL	chronic alcoholism ( osteonecrosis ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Predisposing factors were chronic alcoholism ( osteonecrosis ) and septicemia due to intravenous drug abuse ( suppurative arthritis ) .
	manualset3
130035	3	405423	5	NULL	NULL	0	NULL	septicemia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Predisposing factors were chronic alcoholism ( osteonecrosis ) and septicemia due to intravenous drug abuse ( suppurative arthritis ) .
	manualset3
130036	4	405423	5	NULL	NULL	0	NULL	intravenous drug abuse ( suppurative arthritis )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Predisposing factors were chronic alcoholism ( osteonecrosis ) and septicemia due to intravenous drug abuse ( suppurative arthritis ) .
	manualset3
130037	1	405424	5	NULL	NULL	0	NULL	Predominant VNTR family of strains of Mycobacterium tuberculosis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Predominant VNTR family of strains of Mycobacterium tuberculosis isolated from South Asian patients .
	manualset3
130038	2	405424	5	NULL	NULL	0	NULL	South Asian patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Predominant VNTR family of strains of Mycobacterium tuberculosis isolated from South Asian patients .
	manualset3
130039	1	405425	5	NULL	NULL	0	NULL	constituents 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Predominant constituents of both oils were poly-acetylene esters : ( Z , Z ) - matricaria ester ( 49.4 % and 45.9 % , respectively ) and ( Z ) - lachnophyllum ester ( 37.2 % and 27.5 % , respectively ) , that were accompanied by their stereoisomers as well as appropriate lactones .
	manualset3
130040	2	405425	5	NULL	NULL	0	NULL	oils 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Predominant constituents of both oils were poly-acetylene esters : ( Z , Z ) - matricaria ester ( 49.4 % and 45.9 % , respectively ) and ( Z ) - lachnophyllum ester ( 37.2 % and 27.5 % , respectively ) , that were accompanied by their stereoisomers as well as appropriate lactones .
	manualset3
130041	3	405425	5	NULL	NULL	0	NULL	poly-acetylene esters : ( Z , Z ) - matricaria ester	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Predominant constituents of both oils were poly-acetylene esters : ( Z , Z ) - matricaria ester ( 49.4 % and 45.9 % , respectively ) and ( Z ) - lachnophyllum ester ( 37.2 % and 27.5 % , respectively ) , that were accompanied by their stereoisomers as well as appropriate lactones .
	manualset3
130042	4	405425	5	NULL	NULL	0	NULL	49.4 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Predominant constituents of both oils were poly-acetylene esters : ( Z , Z ) - matricaria ester ( 49.4 % and 45.9 % , respectively ) and ( Z ) - lachnophyllum ester ( 37.2 % and 27.5 % , respectively ) , that were accompanied by their stereoisomers as well as appropriate lactones .
	manualset3
130043	5	405425	5	NULL	NULL	0	NULL	45.9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Predominant constituents of both oils were poly-acetylene esters : ( Z , Z ) - matricaria ester ( 49.4 % and 45.9 % , respectively ) and ( Z ) - lachnophyllum ester ( 37.2 % and 27.5 % , respectively ) , that were accompanied by their stereoisomers as well as appropriate lactones .
	manualset3
130044	6	405425	5	NULL	NULL	0	NULL	( Z ) - lachnophyllum ester	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Predominant constituents of both oils were poly-acetylene esters : ( Z , Z ) - matricaria ester ( 49.4 % and 45.9 % , respectively ) and ( Z ) - lachnophyllum ester ( 37.2 % and 27.5 % , respectively ) , that were accompanied by their stereoisomers as well as appropriate lactones .
	manualset3
130045	7	405425	5	NULL	NULL	0	NULL	37.2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Predominant constituents of both oils were poly-acetylene esters : ( Z , Z ) - matricaria ester ( 49.4 % and 45.9 % , respectively ) and ( Z ) - lachnophyllum ester ( 37.2 % and 27.5 % , respectively ) , that were accompanied by their stereoisomers as well as appropriate lactones .
	manualset3
130046	8	405425	5	NULL	NULL	0	NULL	27.5 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Predominant constituents of both oils were poly-acetylene esters : ( Z , Z ) - matricaria ester ( 49.4 % and 45.9 % , respectively ) and ( Z ) - lachnophyllum ester ( 37.2 % and 27.5 % , respectively ) , that were accompanied by their stereoisomers as well as appropriate lactones .
	manualset3
130047	9	405425	5	NULL	NULL	0	NULL	stereoisomers 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Predominant constituents of both oils were poly-acetylene esters : ( Z , Z ) - matricaria ester ( 49.4 % and 45.9 % , respectively ) and ( Z ) - lachnophyllum ester ( 37.2 % and 27.5 % , respectively ) , that were accompanied by their stereoisomers as well as appropriate lactones .
	manualset3
130048	10	405425	5	NULL	NULL	0	NULL	lactones 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Predominant constituents of both oils were poly-acetylene esters : ( Z , Z ) - matricaria ester ( 49.4 % and 45.9 % , respectively ) and ( Z ) - lachnophyllum ester ( 37.2 % and 27.5 % , respectively ) , that were accompanied by their stereoisomers as well as appropriate lactones .
	manualset3
130049	2	405426	5	NULL	NULL	NULL	NULL	emotional face stimuli	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Preferential processing of emotional face stimuli , however , should elicit sustained neural processing such that repetition suppression to repeated emotional faces is attenuated relative to faces with no emotional content .
	manualset3
130050	1	405426	5	NULL	NULL	0	NULL	Preferential processing 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Preferential processing of emotional face stimuli , however , should elicit sustained neural processing such that repetition suppression to repeated emotional faces is attenuated relative to faces with no emotional content .
	manualset3
130051	3	405426	5	NULL	NULL	0	NULL	sustained neural processing 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Preferential processing of emotional face stimuli , however , should elicit sustained neural processing such that repetition suppression to repeated emotional faces is attenuated relative to faces with no emotional content .
	manualset3
130052	4	405426	5	NULL	NULL	0	NULL	repetition suppression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Preferential processing of emotional face stimuli , however , should elicit sustained neural processing such that repetition suppression to repeated emotional faces is attenuated relative to faces with no emotional content .
	manualset3
130053	5	405426	5	NULL	NULL	0	NULL	emotional faces	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Preferential processing of emotional face stimuli , however , should elicit sustained neural processing such that repetition suppression to repeated emotional faces is attenuated relative to faces with no emotional content .
	manualset3
130054	6	405426	5	NULL	NULL	0	NULL	faces 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Preferential processing of emotional face stimuli , however , should elicit sustained neural processing such that repetition suppression to repeated emotional faces is attenuated relative to faces with no emotional content .
	manualset3
130055	7	405426	5	NULL	NULL	0	NULL	emotional content 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Preferential processing of emotional face stimuli , however , should elicit sustained neural processing such that repetition suppression to repeated emotional faces is attenuated relative to faces with no emotional content .
	manualset3
130056	1	405427	5	NULL	NULL	0	NULL	Pregnancy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnancy and immunosuppressive drug therapy .
	manualset3
130057	2	405427	5	NULL	NULL	0	NULL	immunosuppressive drug therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnancy and immunosuppressive drug therapy .
	manualset3
130058	1	405428	5	NULL	NULL	0	NULL	large number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A large number of cells containing serotonin ( 5-HT ) in the B2 and B6 areas were labeled by FB , while only a few FB-labeled 5-HT cells in B8 , B9 were seen .
	manualset3
130059	2	405428	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A large number of cells containing serotonin ( 5-HT ) in the B2 and B6 areas were labeled by FB , while only a few FB-labeled 5-HT cells in B8 , B9 were seen .
	manualset3
130060	3	405428	5	NULL	NULL	0	NULL	serotonin ( 5-HT )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A large number of cells containing serotonin ( 5-HT ) in the B2 and B6 areas were labeled by FB , while only a few FB-labeled 5-HT cells in B8 , B9 were seen .
	manualset3
130061	4	405428	5	NULL	NULL	NULL	NULL	B2 and B6 areas	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A large number of cells containing serotonin ( 5-HT ) in the B2 and B6 areas were labeled by FB , while only a few FB-labeled 5-HT cells in B8 , B9 were seen .
	manualset3
130062	5	405428	5	NULL	NULL	0	NULL	FB 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A large number of cells containing serotonin ( 5-HT ) in the B2 and B6 areas were labeled by FB , while only a few FB-labeled 5-HT cells in B8 , B9 were seen .
	manualset3
130063	6	405428	5	NULL	NULL	0	NULL	FB-labeled 5-HT cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A large number of cells containing serotonin ( 5-HT ) in the B2 and B6 areas were labeled by FB , while only a few FB-labeled 5-HT cells in B8 , B9 were seen .
	manualset3
130064	7	405428	5	NULL	NULL	0	NULL	B8	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A large number of cells containing serotonin ( 5-HT ) in the B2 and B6 areas were labeled by FB , while only a few FB-labeled 5-HT cells in B8 , B9 were seen .
	manualset3
130065	8	405428	5	NULL	NULL	0	NULL	B9	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A large number of cells containing serotonin ( 5-HT ) in the B2 and B6 areas were labeled by FB , while only a few FB-labeled 5-HT cells in B8 , B9 were seen .
	manualset3
130066	1	405429	5	NULL	NULL	0	NULL	Pregnancy diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnancy diagnosis by repeated rectal palpation and qualitative tests for PMSG , showed that ninety-five mares conceived of which forty-four aborted spontaneously between Days 30 and 160 of gestation .
	manualset3
130067	2	405429	5	NULL	NULL	0	NULL	rectal palpation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnancy diagnosis by repeated rectal palpation and qualitative tests for PMSG , showed that ninety-five mares conceived of which forty-four aborted spontaneously between Days 30 and 160 of gestation .
	manualset3
130068	3	405429	5	NULL	NULL	0	NULL	qualitative tests	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnancy diagnosis by repeated rectal palpation and qualitative tests for PMSG , showed that ninety-five mares conceived of which forty-four aborted spontaneously between Days 30 and 160 of gestation .
	manualset3
130069	4	405429	5	NULL	NULL	0	NULL	PMSG 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnancy diagnosis by repeated rectal palpation and qualitative tests for PMSG , showed that ninety-five mares conceived of which forty-four aborted spontaneously between Days 30 and 160 of gestation .
	manualset3
130070	5	405429	5	NULL	NULL	0	NULL	ninety-five	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnancy diagnosis by repeated rectal palpation and qualitative tests for PMSG , showed that ninety-five mares conceived of which forty-four aborted spontaneously between Days 30 and 160 of gestation .
	manualset3
130071	6	405429	5	NULL	NULL	0	NULL	mares 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnancy diagnosis by repeated rectal palpation and qualitative tests for PMSG , showed that ninety-five mares conceived of which forty-four aborted spontaneously between Days 30 and 160 of gestation .
	manualset3
130072	7	405429	5	NULL	NULL	0	NULL	forty-four	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnancy diagnosis by repeated rectal palpation and qualitative tests for PMSG , showed that ninety-five mares conceived of which forty-four aborted spontaneously between Days 30 and 160 of gestation .
	manualset3
130073	8	405429	5	NULL	NULL	0	NULL	Days 30 and 160	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnancy diagnosis by repeated rectal palpation and qualitative tests for PMSG , showed that ninety-five mares conceived of which forty-four aborted spontaneously between Days 30 and 160 of gestation .
	manualset3
130074	9	405429	5	NULL	NULL	0	NULL	gestation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnancy diagnosis by repeated rectal palpation and qualitative tests for PMSG , showed that ninety-five mares conceived of which forty-four aborted spontaneously between Days 30 and 160 of gestation .
	manualset3
130075	1	405430	5	NULL	NULL	NULL	NULL	Pregnancy 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pregnancy is characterized by a complex interplay of inflammatory events regulated by both the innate and acquired immune systems .
	manualset3
130076	2	405430	5	NULL	NULL	0	NULL	complex interplay 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnancy is characterized by a complex interplay of inflammatory events regulated by both the innate and acquired immune systems .
	manualset3
130077	3	405430	5	NULL	NULL	0	NULL	inflammatory events	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnancy is characterized by a complex interplay of inflammatory events regulated by both the innate and acquired immune systems .
	manualset3
130078	4	405430	5	NULL	NULL	0	NULL	innate immune system	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnancy is characterized by a complex interplay of inflammatory events regulated by both the innate and acquired immune systems .
	manualset3
130079	5	405430	5	NULL	NULL	0	NULL	acquired immune system	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnancy is characterized by a complex interplay of inflammatory events regulated by both the innate and acquired immune systems .
	manualset3
130080	1	405431	5	NULL	NULL	0	NULL	pregnant ewes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnant and nonpregnant ewes were injected with luteinizing hormone-releasing hormone ( LHRH ) .
	manualset3
130081	2	405431	5	NULL	NULL	0	NULL	nonpregnant ewes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnant and nonpregnant ewes were injected with luteinizing hormone-releasing hormone ( LHRH ) .
	manualset3
130082	3	405431	5	NULL	NULL	0	NULL	luteinizing hormone-releasing hormone ( LHRH )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnant and nonpregnant ewes were injected with luteinizing hormone-releasing hormone ( LHRH ) .
	manualset3
130083	1	405432	5	NULL	NULL	0	NULL	Prehypertension 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prehypertension and risk of cardiovascular disease .
	manualset3
130084	2	405432	5	NULL	NULL	0	NULL	risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prehypertension and risk of cardiovascular disease .
	manualset3
130085	3	405432	5	NULL	NULL	0	NULL	cardiovascular disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Prehypertension and risk of cardiovascular disease .
	manualset3
130086	1	405433	5	NULL	NULL	0	NULL	Preincubation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preincubation under conditions in which the high-affinity sites were saturated did not result in stimulation of the calcium uptake rate indicative of closure of the calcium channel .
	manualset3
130087	2	405433	5	NULL	NULL	0	NULL	conditions 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Preincubation under conditions in which the high-affinity sites were saturated did not result in stimulation of the calcium uptake rate indicative of closure of the calcium channel .
	manualset3
130088	3	405433	5	NULL	NULL	NULL	NULL	high-affinity sites	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Preincubation under conditions in which the high-affinity sites were saturated did not result in stimulation of the calcium uptake rate indicative of closure of the calcium channel .
	manualset3
130090	5	405433	5	NULL	NULL	0	NULL	stimulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Preincubation under conditions in which the high-affinity sites were saturated did not result in stimulation of the calcium uptake rate indicative of closure of the calcium channel .
	manualset3
130091	6	405433	5	NULL	NULL	0	NULL	calcium uptake rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preincubation under conditions in which the high-affinity sites were saturated did not result in stimulation of the calcium uptake rate indicative of closure of the calcium channel .
	manualset3
130092	7	405433	5	NULL	NULL	0	NULL	calcium channel	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Preincubation under conditions in which the high-affinity sites were saturated did not result in stimulation of the calcium uptake rate indicative of closure of the calcium channel .
	manualset3
130093	1	405434	5	NULL	NULL	0	NULL	Prelicensing studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Prelicensing studies of vaccines are not specifically designed to detect adverse vaccine reactions .
	manualset3
130094	2	405434	5	NULL	NULL	0	NULL	vaccines 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Prelicensing studies of vaccines are not specifically designed to detect adverse vaccine reactions .
	manualset3
130095	3	405434	5	NULL	NULL	0	NULL	adverse vaccine reactions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prelicensing studies of vaccines are not specifically designed to detect adverse vaccine reactions .
	manualset3
130096	1	405435	5	NULL	NULL	0	NULL	Preliminary analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary analysis of thylakoid membranes with this analytical system gave the PhQ/Chl a ' ratio of 0.58 + / - 0.03 ( n = 4 ) , in line with the stoichiometry of one molecule of Chl a ' per PS I .
	manualset3
130097	2	405435	5	NULL	NULL	0	NULL	thylakoid membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary analysis of thylakoid membranes with this analytical system gave the PhQ/Chl a ' ratio of 0.58 + / - 0.03 ( n = 4 ) , in line with the stoichiometry of one molecule of Chl a ' per PS I .
	manualset3
130098	3	405435	5	NULL	NULL	0	NULL	analytical system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary analysis of thylakoid membranes with this analytical system gave the PhQ/Chl a ' ratio of 0.58 + / - 0.03 ( n = 4 ) , in line with the stoichiometry of one molecule of Chl a ' per PS I .
	manualset3
130099	4	405435	5	NULL	NULL	0	NULL	PhQ/Chl a ' ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary analysis of thylakoid membranes with this analytical system gave the PhQ/Chl a ' ratio of 0.58 + / - 0.03 ( n = 4 ) , in line with the stoichiometry of one molecule of Chl a ' per PS I .
	manualset3
130100	5	405435	5	NULL	NULL	0	NULL	 0.58 + / - 0.03 ( n = 4 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary analysis of thylakoid membranes with this analytical system gave the PhQ/Chl a ' ratio of 0.58 + / - 0.03 ( n = 4 ) , in line with the stoichiometry of one molecule of Chl a ' per PS I .
	manualset3
130101	6	405435	5	NULL	NULL	0	NULL	stoichiometry 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary analysis of thylakoid membranes with this analytical system gave the PhQ/Chl a ' ratio of 0.58 + / - 0.03 ( n = 4 ) , in line with the stoichiometry of one molecule of Chl a ' per PS I .
	manualset3
130102	7	405435	5	NULL	NULL	0	NULL	one molecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary analysis of thylakoid membranes with this analytical system gave the PhQ/Chl a ' ratio of 0.58 + / - 0.03 ( n = 4 ) , in line with the stoichiometry of one molecule of Chl a ' per PS I .
	manualset3
130103	8	405435	5	NULL	NULL	0	NULL	Chl a '	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary analysis of thylakoid membranes with this analytical system gave the PhQ/Chl a ' ratio of 0.58 + / - 0.03 ( n = 4 ) , in line with the stoichiometry of one molecule of Chl a ' per PS I .
	manualset3
130104	9	405435	5	NULL	NULL	0	NULL	PS I	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary analysis of thylakoid membranes with this analytical system gave the PhQ/Chl a ' ratio of 0.58 + / - 0.03 ( n = 4 ) , in line with the stoichiometry of one molecule of Chl a ' per PS I .
	manualset3
130105	1	405436	5	NULL	NULL	0	NULL	large number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A large number of lung nodules remains undetermined after bronchoscopy , radiological and CT imaging analysis .
	manualset3
130106	2	405436	5	NULL	NULL	0	NULL	lung nodules	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A large number of lung nodules remains undetermined after bronchoscopy , radiological and CT imaging analysis .
	manualset3
130107	3	405436	5	NULL	NULL	0	NULL	bronchoscopy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A large number of lung nodules remains undetermined after bronchoscopy , radiological and CT imaging analysis .
	manualset3
130108	4	405436	5	NULL	NULL	NULL	NULL	radiological analysis	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A large number of lung nodules remains undetermined after bronchoscopy , radiological and CT imaging analysis .
	manualset3
134859	5	405436	5	NULL	NULL	0	NULL	CT imaging analysis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A large number of lung nodules remains undetermined after bronchoscopy , radiological and CT imaging analysis .
	manualset3
130109	1	405437	5	NULL	NULL	0	NULL	Preliminary analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary analysis of transgenic mouse brains indicates that expression of double-mutant E22Q/D23N Dutch/Iowa AbetaPP leads to robust deposition of Abeta in a vascular-weighted manner .
	manualset3
130110	2	405437	5	NULL	NULL	0	NULL	transgenic mouse brains	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary analysis of transgenic mouse brains indicates that expression of double-mutant E22Q/D23N Dutch/Iowa AbetaPP leads to robust deposition of Abeta in a vascular-weighted manner .
	manualset3
130111	3	405437	5	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary analysis of transgenic mouse brains indicates that expression of double-mutant E22Q/D23N Dutch/Iowa AbetaPP leads to robust deposition of Abeta in a vascular-weighted manner .
	manualset3
130112	4	405437	5	NULL	NULL	0	NULL	double-mutant E22Q/D23N Dutch/Iowa AbetaPP 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary analysis of transgenic mouse brains indicates that expression of double-mutant E22Q/D23N Dutch/Iowa AbetaPP leads to robust deposition of Abeta in a vascular-weighted manner .
	manualset3
130113	5	405437	5	NULL	NULL	0	NULL	robust deposition 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary analysis of transgenic mouse brains indicates that expression of double-mutant E22Q/D23N Dutch/Iowa AbetaPP leads to robust deposition of Abeta in a vascular-weighted manner .
	manualset3
130114	6	405437	5	NULL	NULL	0	NULL	Abeta 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary analysis of transgenic mouse brains indicates that expression of double-mutant E22Q/D23N Dutch/Iowa AbetaPP leads to robust deposition of Abeta in a vascular-weighted manner .
	manualset3
130115	7	405437	5	NULL	NULL	0	NULL	vascular-weighted manner	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary analysis of transgenic mouse brains indicates that expression of double-mutant E22Q/D23N Dutch/Iowa AbetaPP leads to robust deposition of Abeta in a vascular-weighted manner .
	manualset3
130116	1	405438	5	NULL	NULL	0	NULL	Preliminary costectomy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary costectomy before Harrington instrumentation and fusion for idiopathic scoliosis allows direct excision of the rib prominence and better correction at the second-stage operation .
	manualset3
130117	2	405438	5	NULL	NULL	0	NULL	Harrington instrumentation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary costectomy before Harrington instrumentation and fusion for idiopathic scoliosis allows direct excision of the rib prominence and better correction at the second-stage operation .
	manualset3
130118	3	405438	5	NULL	NULL	0	NULL	fusion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary costectomy before Harrington instrumentation and fusion for idiopathic scoliosis allows direct excision of the rib prominence and better correction at the second-stage operation .
	manualset3
130119	4	405438	5	NULL	NULL	0	NULL	idiopathic scoliosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary costectomy before Harrington instrumentation and fusion for idiopathic scoliosis allows direct excision of the rib prominence and better correction at the second-stage operation .
	manualset3
130120	5	405438	5	NULL	NULL	0	NULL	direct excision	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary costectomy before Harrington instrumentation and fusion for idiopathic scoliosis allows direct excision of the rib prominence and better correction at the second-stage operation .
	manualset3
130121	6	405438	5	NULL	NULL	0	NULL	rib prominence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary costectomy before Harrington instrumentation and fusion for idiopathic scoliosis allows direct excision of the rib prominence and better correction at the second-stage operation .
	manualset3
130122	7	405438	5	NULL	NULL	0	NULL	correction 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary costectomy before Harrington instrumentation and fusion for idiopathic scoliosis allows direct excision of the rib prominence and better correction at the second-stage operation .
	manualset3
130123	8	405438	5	NULL	NULL	0	NULL	second-stage operation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary costectomy before Harrington instrumentation and fusion for idiopathic scoliosis allows direct excision of the rib prominence and better correction at the second-stage operation .
	manualset3
130124	1	405439	5	NULL	NULL	0	NULL	Preliminary data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary data show effective suppression of oestradiol levels in males treated with AI and some reports have demonstrated objective responses .
	manualset3
130125	2	405439	5	NULL	NULL	0	NULL	 effective suppression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary data show effective suppression of oestradiol levels in males treated with AI and some reports have demonstrated objective responses .
	manualset3
130126	3	405439	5	NULL	NULL	0	NULL	oestradiol levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary data show effective suppression of oestradiol levels in males treated with AI and some reports have demonstrated objective responses .
	manualset3
130127	4	405439	5	NULL	NULL	0	NULL	males	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary data show effective suppression of oestradiol levels in males treated with AI and some reports have demonstrated objective responses .
	manualset3
130128	5	405439	5	NULL	NULL	0	NULL	AI	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary data show effective suppression of oestradiol levels in males treated with AI and some reports have demonstrated objective responses .
	manualset3
130129	6	405439	5	NULL	NULL	0	NULL	reports 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary data show effective suppression of oestradiol levels in males treated with AI and some reports have demonstrated objective responses .
	manualset3
130130	7	405439	5	NULL	NULL	0	NULL	objective responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary data show effective suppression of oestradiol levels in males treated with AI and some reports have demonstrated objective responses .
	manualset3
130131	1	405440	5	NULL	NULL	NULL	NULL	Preliminary evaluation	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Preliminary evaluation of sensititre system for identifying gram-negative bacilli .
	manualset3
130132	2	405440	5	NULL	NULL	0	NULL	sensititre system	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary evaluation of sensititre system for identifying gram-negative bacilli .
	manualset3
130133	3	405440	5	NULL	NULL	0	NULL	gram-negative bacilli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary evaluation of sensititre system for identifying gram-negative bacilli .
	manualset3
130134	1	405441	5	NULL	NULL	0	NULL	Preliminary evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary evidence from two phase III , randomized , double-blind , placebo-controlled studies suggest that roflumilast improves or stabilizes lung function , as measured by forced expiratory volume in 1 s and 6 s ( FEV ( 1 ) and FEV ( 6 ) ) , forced vital capacity ( FVC ) , and peak expiratory flow ( PEF ) in patients with COPD .
	manualset3
130135	2	405441	5	NULL	NULL	0	NULL	two phase III , randomized , double-blind , placebo-controlled studies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary evidence from two phase III , randomized , double-blind , placebo-controlled studies suggest that roflumilast improves or stabilizes lung function , as measured by forced expiratory volume in 1 s and 6 s ( FEV ( 1 ) and FEV ( 6 ) ) , forced vital capacity ( FVC ) , and peak expiratory flow ( PEF ) in patients with COPD .
	manualset3
130136	3	405441	5	NULL	NULL	0	NULL	roflumilast 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary evidence from two phase III , randomized , double-blind , placebo-controlled studies suggest that roflumilast improves or stabilizes lung function , as measured by forced expiratory volume in 1 s and 6 s ( FEV ( 1 ) and FEV ( 6 ) ) , forced vital capacity ( FVC ) , and peak expiratory flow ( PEF ) in patients with COPD .
	manualset3
130137	4	405441	5	NULL	NULL	0	NULL	lung function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary evidence from two phase III , randomized , double-blind , placebo-controlled studies suggest that roflumilast improves or stabilizes lung function , as measured by forced expiratory volume in 1 s and 6 s ( FEV ( 1 ) and FEV ( 6 ) ) , forced vital capacity ( FVC ) , and peak expiratory flow ( PEF ) in patients with COPD .
	manualset3
130138	5	405441	5	NULL	NULL	0	NULL	forced expiratory volume in 1 s ( FEV ( 1 ))	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary evidence from two phase III , randomized , double-blind , placebo-controlled studies suggest that roflumilast improves or stabilizes lung function , as measured by forced expiratory volume in 1 s and 6 s ( FEV ( 1 ) and FEV ( 6 ) ) , forced vital capacity ( FVC ) , and peak expiratory flow ( PEF ) in patients with COPD .
	manualset3
130139	6	405441	5	NULL	NULL	0	NULL	forced expiratory volume in  6 s (FEV ( 6 ) )  	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary evidence from two phase III , randomized , double-blind , placebo-controlled studies suggest that roflumilast improves or stabilizes lung function , as measured by forced expiratory volume in 1 s and 6 s ( FEV ( 1 ) and FEV ( 6 ) ) , forced vital capacity ( FVC ) , and peak expiratory flow ( PEF ) in patients with COPD .
	manualset3
130140	7	405441	5	NULL	NULL	0	NULL	forced vital capacity ( FVC )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary evidence from two phase III , randomized , double-blind , placebo-controlled studies suggest that roflumilast improves or stabilizes lung function , as measured by forced expiratory volume in 1 s and 6 s ( FEV ( 1 ) and FEV ( 6 ) ) , forced vital capacity ( FVC ) , and peak expiratory flow ( PEF ) in patients with COPD .
	manualset3
130141	8	405441	5	NULL	NULL	0	NULL	peak expiratory flow ( PEF )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary evidence from two phase III , randomized , double-blind , placebo-controlled studies suggest that roflumilast improves or stabilizes lung function , as measured by forced expiratory volume in 1 s and 6 s ( FEV ( 1 ) and FEV ( 6 ) ) , forced vital capacity ( FVC ) , and peak expiratory flow ( PEF ) in patients with COPD .
	manualset3
130142	9	405441	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary evidence from two phase III , randomized , double-blind , placebo-controlled studies suggest that roflumilast improves or stabilizes lung function , as measured by forced expiratory volume in 1 s and 6 s ( FEV ( 1 ) and FEV ( 6 ) ) , forced vital capacity ( FVC ) , and peak expiratory flow ( PEF ) in patients with COPD .
	manualset3
130143	10	405441	5	NULL	NULL	0	NULL	COPD 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary evidence from two phase III , randomized , double-blind , placebo-controlled studies suggest that roflumilast improves or stabilizes lung function , as measured by forced expiratory volume in 1 s and 6 s ( FEV ( 1 ) and FEV ( 6 ) ) , forced vital capacity ( FVC ) , and peak expiratory flow ( PEF ) in patients with COPD .
	manualset3
130144	1	405442	5	NULL	NULL	0	NULL	Preliminary experiences	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary experiences with two new antihypertensives : guanethidine and bretylium tosylate .
	manualset3
130145	2	405442	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary experiences with two new antihypertensives : guanethidine and bretylium tosylate .
	manualset3
130146	3	405442	5	NULL	NULL	0	NULL	antihypertensives 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary experiences with two new antihypertensives : guanethidine and bretylium tosylate .
	manualset3
130147	4	405442	5	NULL	NULL	0	NULL	guanethidine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary experiences with two new antihypertensives : guanethidine and bretylium tosylate .
	manualset3
130148	5	405442	5	NULL	NULL	0	NULL	bretylium tosylate	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary experiences with two new antihypertensives : guanethidine and bretylium tosylate .
	manualset3
130149	1	405443	5	NULL	NULL	0	NULL	Preliminary microcalorimetric studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary microcalorimetric studies have been performed to analyze the response of a whole epiphytic lichen tissue ( Evernia prunastri ) to 2-chlorophenol ( 2Cl-phi ) , a pollutant of oil mill waste-water , in order to evaluate whether the tissue might be used to assess the toxic characteristics of polluted waters .
	manualset3
130150	2	405443	5	NULL	NULL	0	NULL	response 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary microcalorimetric studies have been performed to analyze the response of a whole epiphytic lichen tissue ( Evernia prunastri ) to 2-chlorophenol ( 2Cl-phi ) , a pollutant of oil mill waste-water , in order to evaluate whether the tissue might be used to assess the toxic characteristics of polluted waters .
	manualset3
130151	3	405443	5	NULL	NULL	0	NULL	whole epiphytic lichen tissue ( Evernia prunastri )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary microcalorimetric studies have been performed to analyze the response of a whole epiphytic lichen tissue ( Evernia prunastri ) to 2-chlorophenol ( 2Cl-phi ) , a pollutant of oil mill waste-water , in order to evaluate whether the tissue might be used to assess the toxic characteristics of polluted waters .
	manualset3
130152	4	405443	5	NULL	NULL	0	NULL	2-chlorophenol ( 2Cl-phi )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary microcalorimetric studies have been performed to analyze the response of a whole epiphytic lichen tissue ( Evernia prunastri ) to 2-chlorophenol ( 2Cl-phi ) , a pollutant of oil mill waste-water , in order to evaluate whether the tissue might be used to assess the toxic characteristics of polluted waters .
	manualset3
130153	5	405443	5	NULL	NULL	0	NULL	pollutant 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary microcalorimetric studies have been performed to analyze the response of a whole epiphytic lichen tissue ( Evernia prunastri ) to 2-chlorophenol ( 2Cl-phi ) , a pollutant of oil mill waste-water , in order to evaluate whether the tissue might be used to assess the toxic characteristics of polluted waters .
	manualset3
130154	6	405443	5	NULL	NULL	NULL	NULL	oil mill waste-water	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Preliminary microcalorimetric studies have been performed to analyze the response of a whole epiphytic lichen tissue ( Evernia prunastri ) to 2-chlorophenol ( 2Cl-phi ) , a pollutant of oil mill waste-water , in order to evaluate whether the tissue might be used to assess the toxic characteristics of polluted waters .
	manualset3
130155	7	405443	5	NULL	NULL	0	NULL	tissue 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary microcalorimetric studies have been performed to analyze the response of a whole epiphytic lichen tissue ( Evernia prunastri ) to 2-chlorophenol ( 2Cl-phi ) , a pollutant of oil mill waste-water , in order to evaluate whether the tissue might be used to assess the toxic characteristics of polluted waters .
	manualset3
130156	8	405443	5	NULL	NULL	0	NULL	toxic characteristics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary microcalorimetric studies have been performed to analyze the response of a whole epiphytic lichen tissue ( Evernia prunastri ) to 2-chlorophenol ( 2Cl-phi ) , a pollutant of oil mill waste-water , in order to evaluate whether the tissue might be used to assess the toxic characteristics of polluted waters .
	manualset3
130157	9	405443	5	NULL	NULL	0	NULL	polluted waters	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary microcalorimetric studies have been performed to analyze the response of a whole epiphytic lichen tissue ( Evernia prunastri ) to 2-chlorophenol ( 2Cl-phi ) , a pollutant of oil mill waste-water , in order to evaluate whether the tissue might be used to assess the toxic characteristics of polluted waters .
	manualset3
130158	1	405444	5	NULL	NULL	0	NULL	Preliminary observations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary observations on expression of transforming growth factors beta1 and beta3 in equine full-thickness skin wounds healing normally or with exuberant granulation tissue .
	manualset3
130159	2	405444	5	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary observations on expression of transforming growth factors beta1 and beta3 in equine full-thickness skin wounds healing normally or with exuberant granulation tissue .
	manualset3
130160	3	405444	5	NULL	NULL	0	NULL	transforming growth factor beta1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary observations on expression of transforming growth factors beta1 and beta3 in equine full-thickness skin wounds healing normally or with exuberant granulation tissue .
	manualset3
130161	4	405444	5	NULL	NULL	0	NULL	transforming growth factor beta3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary observations on expression of transforming growth factors beta1 and beta3 in equine full-thickness skin wounds healing normally or with exuberant granulation tissue .
	manualset3
130162	5	405444	5	NULL	NULL	0	NULL	equine full-thickness skin wounds	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary observations on expression of transforming growth factors beta1 and beta3 in equine full-thickness skin wounds healing normally or with exuberant granulation tissue .
	manualset3
130163	6	405444	5	NULL	NULL	0	NULL	granulation tissue	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary observations on expression of transforming growth factors beta1 and beta3 in equine full-thickness skin wounds healing normally or with exuberant granulation tissue .
	manualset3
130164	1	405445	5	NULL	NULL	0	NULL	Preliminary results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary results in normal controls and patients with untreated coeliac disease are presented .
	manualset3
130165	2	405445	5	NULL	NULL	0	NULL	normal controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary results in normal controls and patients with untreated coeliac disease are presented .
	manualset3
130166	3	405445	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary results in normal controls and patients with untreated coeliac disease are presented .
	manualset3
130167	4	405445	5	NULL	NULL	0	NULL	untreated coeliac disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary results in normal controls and patients with untreated coeliac disease are presented .
	manualset3
130168	1	405446	5	NULL	NULL	0	NULL	 large number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A large number of studies has been carried out in normal volunteers and patients with a variety of CNS disorders .
	manualset3
130169	2	405446	5	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A large number of studies has been carried out in normal volunteers and patients with a variety of CNS disorders .
	manualset3
130170	3	405446	5	NULL	NULL	0	NULL	normal volunteers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A large number of studies has been carried out in normal volunteers and patients with a variety of CNS disorders .
	manualset3
130171	4	405446	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A large number of studies has been carried out in normal volunteers and patients with a variety of CNS disorders .
	manualset3
130172	5	405446	5	NULL	NULL	0	NULL	CNS disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A large number of studies has been carried out in normal volunteers and patients with a variety of CNS disorders .
	manualset3
130173	1	405447	5	NULL	NULL	0	NULL	Preliminary studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary studies in Alzheimer 's disease have demonstrated elevated levels of phosphomonoesters and phosphodiesters in the areas of Alzheimer 's brain which exhibit neuropathological changes .
	manualset3
130174	2	405447	5	NULL	NULL	0	NULL	Alzheimer 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary studies in Alzheimer 's disease have demonstrated elevated levels of phosphomonoesters and phosphodiesters in the areas of Alzheimer 's brain which exhibit neuropathological changes .
	manualset3
130175	3	405447	5	NULL	NULL	0	NULL	elevated levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary studies in Alzheimer 's disease have demonstrated elevated levels of phosphomonoesters and phosphodiesters in the areas of Alzheimer 's brain which exhibit neuropathological changes .
	manualset3
130176	4	405447	5	NULL	NULL	0	NULL	phosphomonoesters 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary studies in Alzheimer 's disease have demonstrated elevated levels of phosphomonoesters and phosphodiesters in the areas of Alzheimer 's brain which exhibit neuropathological changes .
	manualset3
130177	5	405447	5	NULL	NULL	0	NULL	phosphodiesters 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary studies in Alzheimer 's disease have demonstrated elevated levels of phosphomonoesters and phosphodiesters in the areas of Alzheimer 's brain which exhibit neuropathological changes .
	manualset3
130178	6	405447	5	NULL	NULL	0	NULL	areas 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary studies in Alzheimer 's disease have demonstrated elevated levels of phosphomonoesters and phosphodiesters in the areas of Alzheimer 's brain which exhibit neuropathological changes .
	manualset3
130179	7	405447	5	NULL	NULL	0	NULL	Alzheimer 's brain 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary studies in Alzheimer 's disease have demonstrated elevated levels of phosphomonoesters and phosphodiesters in the areas of Alzheimer 's brain which exhibit neuropathological changes .
	manualset3
130180	8	405447	5	NULL	NULL	0	NULL	neuropathological changes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary studies in Alzheimer 's disease have demonstrated elevated levels of phosphomonoesters and phosphodiesters in the areas of Alzheimer 's brain which exhibit neuropathological changes .
	manualset3
130181	1	405448	5	NULL	NULL	0	NULL	Preliminary studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary studies in rabbits showed that the optimal volume of injected material should be 7.5 times the volume of 1 cm vas segment ; the effective rate was 100 % .
	manualset3
130182	2	405448	5	NULL	NULL	0	NULL	rabbits 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary studies in rabbits showed that the optimal volume of injected material should be 7.5 times the volume of 1 cm vas segment ; the effective rate was 100 % .
	manualset3
130183	3	405448	5	NULL	NULL	0	NULL	optimal volume	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary studies in rabbits showed that the optimal volume of injected material should be 7.5 times the volume of 1 cm vas segment ; the effective rate was 100 % .
	manualset3
130184	4	405448	5	NULL	NULL	0	NULL	injected material	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary studies in rabbits showed that the optimal volume of injected material should be 7.5 times the volume of 1 cm vas segment ; the effective rate was 100 % .
	manualset3
130185	5	405448	5	NULL	NULL	0	NULL	7.5 times	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary studies in rabbits showed that the optimal volume of injected material should be 7.5 times the volume of 1 cm vas segment ; the effective rate was 100 % .
	manualset3
130186	6	405448	5	NULL	NULL	0	NULL	volume 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary studies in rabbits showed that the optimal volume of injected material should be 7.5 times the volume of 1 cm vas segment ; the effective rate was 100 % .
	manualset3
130187	7	405448	5	NULL	NULL	0	NULL	1 cm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary studies in rabbits showed that the optimal volume of injected material should be 7.5 times the volume of 1 cm vas segment ; the effective rate was 100 % .
	manualset3
130188	8	405448	5	NULL	NULL	0	NULL	vas segment	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary studies in rabbits showed that the optimal volume of injected material should be 7.5 times the volume of 1 cm vas segment ; the effective rate was 100 % .
	manualset3
130189	9	405448	5	NULL	NULL	0	NULL	effective rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary studies in rabbits showed that the optimal volume of injected material should be 7.5 times the volume of 1 cm vas segment ; the effective rate was 100 % .
	manualset3
130190	10	405448	5	NULL	NULL	0	NULL	100 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary studies in rabbits showed that the optimal volume of injected material should be 7.5 times the volume of 1 cm vas segment ; the effective rate was 100 % .
	manualset3
130191	1	405449	5	NULL	NULL	0	NULL	Preliminary studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary studies on the use of n-butyl chloride as an extractant in a drug screening procedure .
	manualset3
130192	2	405449	5	NULL	NULL	0	NULL	 n-butyl chloride	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary studies on the use of n-butyl chloride as an extractant in a drug screening procedure .
	manualset3
130193	3	405449	5	NULL	NULL	0	NULL	extractant 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary studies on the use of n-butyl chloride as an extractant in a drug screening procedure .
	manualset3
130194	4	405449	5	NULL	NULL	0	NULL	drug screening procedure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary studies on the use of n-butyl chloride as an extractant in a drug screening procedure .
	manualset3
130195	1	405450	5	NULL	NULL	0	NULL	Preliminary toxicity study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary toxicity study for RG - ( gal ) ( 28 ) GSA using Balb/c mice reveal no toxic effects up to 100x of the standard imaging dose of 1 mg/kg administered either intraperitoneally or intravenously .
	manualset3
130196	2	405450	5	NULL	NULL	0	NULL	RG - ( gal ) ( 28 ) GSA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary toxicity study for RG - ( gal ) ( 28 ) GSA using Balb/c mice reveal no toxic effects up to 100x of the standard imaging dose of 1 mg/kg administered either intraperitoneally or intravenously .
	manualset3
130197	3	405450	5	NULL	NULL	0	NULL	Balb/c mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary toxicity study for RG - ( gal ) ( 28 ) GSA using Balb/c mice reveal no toxic effects up to 100x of the standard imaging dose of 1 mg/kg administered either intraperitoneally or intravenously .
	manualset3
130198	4	405450	5	NULL	NULL	0	NULL	toxic effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary toxicity study for RG - ( gal ) ( 28 ) GSA using Balb/c mice reveal no toxic effects up to 100x of the standard imaging dose of 1 mg/kg administered either intraperitoneally or intravenously .
	manualset3
130199	5	405450	5	NULL	NULL	0	NULL	100x	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary toxicity study for RG - ( gal ) ( 28 ) GSA using Balb/c mice reveal no toxic effects up to 100x of the standard imaging dose of 1 mg/kg administered either intraperitoneally or intravenously .
	manualset3
130200	6	405450	5	NULL	NULL	0	NULL	standard imaging dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary toxicity study for RG - ( gal ) ( 28 ) GSA using Balb/c mice reveal no toxic effects up to 100x of the standard imaging dose of 1 mg/kg administered either intraperitoneally or intravenously .
	manualset3
130201	7	405450	5	NULL	NULL	0	NULL	1 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary toxicity study for RG - ( gal ) ( 28 ) GSA using Balb/c mice reveal no toxic effects up to 100x of the standard imaging dose of 1 mg/kg administered either intraperitoneally or intravenously .
	manualset3
130202	1	405451	5	NULL	NULL	0	NULL	Preliminary work 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary work demonstrated the induction of c-fos and alpha-interferon genes following exposure to low-linear-energy-transfer ( low-LET ) radiations ( X rays or gamma rays ) .
	manualset3
130203	2	405451	5	NULL	NULL	0	NULL	induction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary work demonstrated the induction of c-fos and alpha-interferon genes following exposure to low-linear-energy-transfer ( low-LET ) radiations ( X rays or gamma rays ) .
	manualset3
130204	3	405451	5	NULL	NULL	0	NULL	c-fos	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary work demonstrated the induction of c-fos and alpha-interferon genes following exposure to low-linear-energy-transfer ( low-LET ) radiations ( X rays or gamma rays ) .
	manualset3
130205	4	405451	5	NULL	NULL	0	NULL	alpha-interferon genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary work demonstrated the induction of c-fos and alpha-interferon genes following exposure to low-linear-energy-transfer ( low-LET ) radiations ( X rays or gamma rays ) .
	manualset3
130206	5	405451	5	NULL	NULL	0	NULL	exposure 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary work demonstrated the induction of c-fos and alpha-interferon genes following exposure to low-linear-energy-transfer ( low-LET ) radiations ( X rays or gamma rays ) .
	manualset3
130207	6	405451	5	NULL	NULL	0	NULL	low-linear-energy-transfer ( low-LET ) radiations ( X rays or gamma rays )	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary work demonstrated the induction of c-fos and alpha-interferon genes following exposure to low-linear-energy-transfer ( low-LET ) radiations ( X rays or gamma rays ) .
	manualset3
130208	1	405452	5	NULL	NULL	0	NULL	Premenstrual syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Premenstrual syndrome : a view from the bench .
	manualset3
130209	2	405452	5	NULL	NULL	0	NULL	bench 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Premenstrual syndrome : a view from the bench .
	manualset3
130210	1	405453	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Premise of the study : The stability of the bimodal karyotype found in Agave and closely related species has long interested botanists .
	manualset3
130211	2	405453	5	NULL	NULL	0	NULL	stability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Premise of the study : The stability of the bimodal karyotype found in Agave and closely related species has long interested botanists .
	manualset3
130212	3	405453	5	NULL	NULL	0	NULL	bimodal karyotype	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Premise of the study : The stability of the bimodal karyotype found in Agave and closely related species has long interested botanists .
	manualset3
130213	4	405453	5	NULL	NULL	0	NULL	Agave 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Premise of the study : The stability of the bimodal karyotype found in Agave and closely related species has long interested botanists .
	manualset3
130214	5	405453	5	NULL	NULL	0	NULL	closely related species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Premise of the study : The stability of the bimodal karyotype found in Agave and closely related species has long interested botanists .
	manualset3
130215	6	405453	5	NULL	NULL	0	NULL	 long interested botanists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Premise of the study : The stability of the bimodal karyotype found in Agave and closely related species has long interested botanists .
	manualset3
130216	1	405454	5	NULL	NULL	0	NULL	Prenatal morphine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Prenatal morphine had no effects on NE turnover in the male POA , but in female rats NE turnover decreased approximately 60 % .
	manualset3
130217	2	405454	5	NULL	NULL	0	NULL	NE turnover	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Prenatal morphine had no effects on NE turnover in the male POA , but in female rats NE turnover decreased approximately 60 % .
	manualset3
130218	3	405454	5	NULL	NULL	0	NULL	male POA	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Prenatal morphine had no effects on NE turnover in the male POA , but in female rats NE turnover decreased approximately 60 % .
	manualset3
130219	4	405454	5	NULL	NULL	0	NULL	female rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Prenatal morphine had no effects on NE turnover in the male POA , but in female rats NE turnover decreased approximately 60 % .
	manualset3
130220	5	405454	5	NULL	NULL	0	NULL	NE turnover	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Prenatal morphine had no effects on NE turnover in the male POA , but in female rats NE turnover decreased approximately 60 % .
	manualset3
130221	6	405454	5	NULL	NULL	0	NULL	60 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Prenatal morphine had no effects on NE turnover in the male POA , but in female rats NE turnover decreased approximately 60 % .
	manualset3
130222	1	405455	5	NULL	NULL	0	NULL	Calcium levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Calcium levels and calciuria in decalcification in acromegaly ) .
	manualset3
130223	2	405455	5	NULL	NULL	0	NULL	calciuria 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Calcium levels and calciuria in decalcification in acromegaly ) .
	manualset3
130224	3	405455	5	NULL	NULL	0	NULL	decalcification 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Calcium levels and calciuria in decalcification in acromegaly ) .
	manualset3
130225	4	405455	5	NULL	NULL	0	NULL	acromegaly 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Calcium levels and calciuria in decalcification in acromegaly ) .
	manualset3
130226	1	405456	5	NULL	NULL	0	NULL	Prenatal sonographic diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prenatal sonographic diagnosis of familial Saethre-Chotzen syndrome .
	manualset3
130227	2	405456	5	NULL	NULL	0	NULL	familial Saethre-Chotzen syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Prenatal sonographic diagnosis of familial Saethre-Chotzen syndrome .
	manualset3
130228	1	405457	5	NULL	NULL	0	NULL	dilatation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prenatally or postnatally diagnosed dilatation of the upper urinary tract initiates postnatal investigations , including sonography , dynamic renography ( MAG 3 ) and optional voiding cystourethrography .
	manualset3
130229	2	405457	5	NULL	NULL	0	NULL	upper urinary tract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Prenatally or postnatally diagnosed dilatation of the upper urinary tract initiates postnatal investigations , including sonography , dynamic renography ( MAG 3 ) and optional voiding cystourethrography .
	manualset3
130230	3	405457	5	NULL	NULL	0	NULL	postnatal investigations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prenatally or postnatally diagnosed dilatation of the upper urinary tract initiates postnatal investigations , including sonography , dynamic renography ( MAG 3 ) and optional voiding cystourethrography .
	manualset3
130231	4	405457	5	NULL	NULL	0	NULL	sonography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prenatally or postnatally diagnosed dilatation of the upper urinary tract initiates postnatal investigations , including sonography , dynamic renography ( MAG 3 ) and optional voiding cystourethrography .
	manualset3
130232	5	405457	5	NULL	NULL	0	NULL	dynamic renography ( MAG 3 ) 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prenatally or postnatally diagnosed dilatation of the upper urinary tract initiates postnatal investigations , including sonography , dynamic renography ( MAG 3 ) and optional voiding cystourethrography .
	manualset3
130233	6	405457	5	NULL	NULL	0	NULL	optional voiding cystourethrography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prenatally or postnatally diagnosed dilatation of the upper urinary tract initiates postnatal investigations , including sonography , dynamic renography ( MAG 3 ) and optional voiding cystourethrography .
	manualset3
130234	1	405458	5	NULL	NULL	0	NULL	Prenylated protein methyltransferase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Prenylated protein methyltransferase , an enzyme involved in the post-translational modification of many signalling proteins , has been characterized in a parasitic flagellated protozoan , Leishmania donovani .
	manualset3
130235	2	405458	5	NULL	NULL	0	NULL	enzyme 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Prenylated protein methyltransferase , an enzyme involved in the post-translational modification of many signalling proteins , has been characterized in a parasitic flagellated protozoan , Leishmania donovani .
	manualset3
130236	3	405458	5	NULL	NULL	0	NULL	post-translational modification	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Prenylated protein methyltransferase , an enzyme involved in the post-translational modification of many signalling proteins , has been characterized in a parasitic flagellated protozoan , Leishmania donovani .
	manualset3
130237	4	405458	5	NULL	NULL	0	NULL	signalling proteins	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Prenylated protein methyltransferase , an enzyme involved in the post-translational modification of many signalling proteins , has been characterized in a parasitic flagellated protozoan , Leishmania donovani .
	manualset3
130238	5	405458	5	NULL	NULL	0	NULL	parasitic flagellated protozoan , Leishmania donovani	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Prenylated protein methyltransferase , an enzyme involved in the post-translational modification of many signalling proteins , has been characterized in a parasitic flagellated protozoan , Leishmania donovani .
	manualset3
130239	1	405459	5	NULL	NULL	0	NULL	Preoperative angiographic localization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Preoperative angiographic localization of insulin-producing tumors of the pancreas .
	manualset3
130240	2	405459	5	NULL	NULL	0	NULL	 insulin-producing tumors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Preoperative angiographic localization of insulin-producing tumors of the pancreas .
	manualset3
130241	3	405459	5	NULL	NULL	0	NULL	pancreas 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Preoperative angiographic localization of insulin-producing tumors of the pancreas .
	manualset3
130242	1	405460	5	NULL	NULL	0	NULL	Preoperative radiologic assessment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Preoperative radiologic assessment should evaluate the status of the middle/inner ear , auditory nerve and central acoustic pathways .
	manualset3
130243	2	405460	5	NULL	NULL	0	NULL	status 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preoperative radiologic assessment should evaluate the status of the middle/inner ear , auditory nerve and central acoustic pathways .
	manualset3
130244	3	405460	5	NULL	NULL	0	NULL	middle/inner ear	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Preoperative radiologic assessment should evaluate the status of the middle/inner ear , auditory nerve and central acoustic pathways .
	manualset3
130245	4	405460	5	NULL	NULL	0	NULL	auditory nerve	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Preoperative radiologic assessment should evaluate the status of the middle/inner ear , auditory nerve and central acoustic pathways .
	manualset3
130246	5	405460	5	NULL	NULL	0	NULL	central acoustic pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Preoperative radiologic assessment should evaluate the status of the middle/inner ear , auditory nerve and central acoustic pathways .
	manualset3
130247	1	405461	5	NULL	NULL	0	NULL	Preparation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Preparation and physicochemical characterization of amoxicillin beta-cyclodextrin complexes .
	manualset3
130248	2	405461	5	NULL	NULL	0	NULL	physicochemical characterization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preparation and physicochemical characterization of amoxicillin beta-cyclodextrin complexes .
	manualset3
130249	3	405461	5	NULL	NULL	0	NULL	amoxicillin beta-cyclodextrin complexes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Preparation and physicochemical characterization of amoxicillin beta-cyclodextrin complexes .
	manualset3
130250	1	405462	5	NULL	NULL	0	NULL	Preparation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preparation of PHA granules by discontinuous density gradient centrifugation of crude cellular extracts revealed four major bands in an SDS polyacrylamide gel .
	manualset3
130251	2	405462	5	NULL	NULL	0	NULL	PHA granules	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Preparation of PHA granules by discontinuous density gradient centrifugation of crude cellular extracts revealed four major bands in an SDS polyacrylamide gel .
	manualset3
130252	3	405462	5	NULL	NULL	0	NULL	discontinuous density gradient centrifugation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preparation of PHA granules by discontinuous density gradient centrifugation of crude cellular extracts revealed four major bands in an SDS polyacrylamide gel .
	manualset3
130253	4	405462	5	NULL	NULL	0	NULL	crude cellular extracts 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Preparation of PHA granules by discontinuous density gradient centrifugation of crude cellular extracts revealed four major bands in an SDS polyacrylamide gel .
	manualset3
130254	5	405462	5	NULL	NULL	0	NULL	four 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Preparation of PHA granules by discontinuous density gradient centrifugation of crude cellular extracts revealed four major bands in an SDS polyacrylamide gel .
	manualset3
130255	6	405462	5	NULL	NULL	0	NULL	major bands	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preparation of PHA granules by discontinuous density gradient centrifugation of crude cellular extracts revealed four major bands in an SDS polyacrylamide gel .
	manualset3
130256	7	405462	5	NULL	NULL	0	NULL	SDS polyacrylamide gel 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Preparation of PHA granules by discontinuous density gradient centrifugation of crude cellular extracts revealed four major bands in an SDS polyacrylamide gel .
	manualset3
130257	1	405463	5	NULL	NULL	0	NULL	large proportion	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A large proportion ( 33 % ) of isolates harbored double mutant dhfr genotype ( 51I , 59 C , 108 N ) .
	manualset3
130258	2	405463	5	NULL	NULL	0	NULL	33 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A large proportion ( 33 % ) of isolates harbored double mutant dhfr genotype ( 51I , 59 C , 108 N ) .
	manualset3
130259	3	405463	5	NULL	NULL	0	NULL	isolates 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A large proportion ( 33 % ) of isolates harbored double mutant dhfr genotype ( 51I , 59 C , 108 N ) .
	manualset3
130260	4	405463	5	NULL	NULL	0	NULL	double mutant dhfr genotype ( 51I , 59 C , 108 N )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A large proportion ( 33 % ) of isolates harbored double mutant dhfr genotype ( 51I , 59 C , 108 N ) .
	manualset3
130261	1	405464	5	NULL	NULL	0	NULL	Preparation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preparation of di and tri ( bis ( indolyl ) methanes ) from di and trialdehydes and indoles in the presence of silica sulfuric acid was described .
	manualset3
130262	2	405464	5	NULL	NULL	0	NULL	di and tri ( bis ( indolyl ) methanes )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Preparation of di and tri ( bis ( indolyl ) methanes ) from di and trialdehydes and indoles in the presence of silica sulfuric acid was described .
	manualset3
130263	3	405464	5	NULL	NULL	0	NULL	di and trialdehydes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Preparation of di and tri ( bis ( indolyl ) methanes ) from di and trialdehydes and indoles in the presence of silica sulfuric acid was described .
	manualset3
130264	4	405464	5	NULL	NULL	0	NULL	indoles 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Preparation of di and tri ( bis ( indolyl ) methanes ) from di and trialdehydes and indoles in the presence of silica sulfuric acid was described .
	manualset3
130265	5	405464	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Preparation of di and tri ( bis ( indolyl ) methanes ) from di and trialdehydes and indoles in the presence of silica sulfuric acid was described .
	manualset3
130266	6	405464	5	NULL	NULL	0	NULL	silica sulfuric acid	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Preparation of di and tri ( bis ( indolyl ) methanes ) from di and trialdehydes and indoles in the presence of silica sulfuric acid was described .
	manualset3
130267	1	405465	5	NULL	NULL	0	NULL	future 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Preparing for the future : perianesthesia orientation .
	manualset3
130268	2	405465	5	NULL	NULL	0	NULL	perianesthesia orientation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Preparing for the future : perianesthesia orientation .
	manualset3
130269	1	405466	5	NULL	NULL	0	NULL	Prephenate 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Prephenate and chorismate , as well as a number of naturally occurring phenazine compounds , inhibited the DAHP synthetase activity to varying degrees .
	manualset3
130270	2	405466	5	NULL	NULL	0	NULL	chorismate 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Prephenate and chorismate , as well as a number of naturally occurring phenazine compounds , inhibited the DAHP synthetase activity to varying degrees .
	manualset3
130271	3	405466	5	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Prephenate and chorismate , as well as a number of naturally occurring phenazine compounds , inhibited the DAHP synthetase activity to varying degrees .
	manualset3
130272	4	405466	5	NULL	NULL	0	NULL	naturally occurring phenazine compounds	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Prephenate and chorismate , as well as a number of naturally occurring phenazine compounds , inhibited the DAHP synthetase activity to varying degrees .
	manualset3
130273	5	405466	5	NULL	NULL	0	NULL	DAHP synthetase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Prephenate and chorismate , as well as a number of naturally occurring phenazine compounds , inhibited the DAHP synthetase activity to varying degrees .
	manualset3
130274	6	405466	5	NULL	NULL	0	NULL	varying degrees	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Prephenate and chorismate , as well as a number of naturally occurring phenazine compounds , inhibited the DAHP synthetase activity to varying degrees .
	manualset3
130275	1	405467	5	NULL	NULL	NULL	NULL	Prepubertal rats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Prepubertal and 13-month-old rats were adrenalectomized ( ADX ) or sham operated ( SHAM ) .
	manualset3
130276	2	405467	5	NULL	NULL	0	NULL	13-month-old rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Prepubertal and 13-month-old rats were adrenalectomized ( ADX ) or sham operated ( SHAM ) .
	manualset3
130277	1	405468	5	NULL	NULL	0	NULL	Prerequisites 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Prerequisites for effective condom promotion campaigns .
	manualset3
130278	2	405468	5	NULL	NULL	0	NULL	condom promotion campaigns 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prerequisites for effective condom promotion campaigns .
	manualset3
130279	1	405469	5	NULL	NULL	0	NULL	Presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of BrdU ( 0.8 microM ) for more than one cell cycle ( 24 hr ) significantly increased gamma-ray ( 1-4 Gy ) induced micronuclei formation in exponentially growing BMG-1 cells .
	manualset3
130280	2	405469	5	NULL	NULL	0	NULL	BrdU 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of BrdU ( 0.8 microM ) for more than one cell cycle ( 24 hr ) significantly increased gamma-ray ( 1-4 Gy ) induced micronuclei formation in exponentially growing BMG-1 cells .
	manualset3
130281	3	405469	5	NULL	NULL	0	NULL	0.8 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of BrdU ( 0.8 microM ) for more than one cell cycle ( 24 hr ) significantly increased gamma-ray ( 1-4 Gy ) induced micronuclei formation in exponentially growing BMG-1 cells .
	manualset3
130282	4	405469	5	NULL	NULL	0	NULL	one cell cycle	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of BrdU ( 0.8 microM ) for more than one cell cycle ( 24 hr ) significantly increased gamma-ray ( 1-4 Gy ) induced micronuclei formation in exponentially growing BMG-1 cells .
	manualset3
130283	5	405469	5	NULL	NULL	0	NULL	 24 hr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of BrdU ( 0.8 microM ) for more than one cell cycle ( 24 hr ) significantly increased gamma-ray ( 1-4 Gy ) induced micronuclei formation in exponentially growing BMG-1 cells .
	manualset3
130284	6	405469	5	NULL	NULL	0	NULL	gamma-ray ( 1-4 Gy )	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of BrdU ( 0.8 microM ) for more than one cell cycle ( 24 hr ) significantly increased gamma-ray ( 1-4 Gy ) induced micronuclei formation in exponentially growing BMG-1 cells .
	manualset3
130285	7	405469	5	NULL	NULL	0	NULL	micronuclei formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of BrdU ( 0.8 microM ) for more than one cell cycle ( 24 hr ) significantly increased gamma-ray ( 1-4 Gy ) induced micronuclei formation in exponentially growing BMG-1 cells .
	manualset3
130286	8	405469	5	NULL	NULL	0	NULL	BMG-1 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of BrdU ( 0.8 microM ) for more than one cell cycle ( 24 hr ) significantly increased gamma-ray ( 1-4 Gy ) induced micronuclei formation in exponentially growing BMG-1 cells .
	manualset3
130287	1	405470	5	NULL	NULL	0	NULL	large tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A large tumor measuring 9.2 x 8.4 cm was observed in the posterior wall of the upper portion of the stomach .
	manualset3
130288	2	405470	5	NULL	NULL	0	NULL	9.2 x 8.4 cm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A large tumor measuring 9.2 x 8.4 cm was observed in the posterior wall of the upper portion of the stomach .
	manualset3
130289	3	405470	5	NULL	NULL	0	NULL	posterior wall of the upper portion of the stomach	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A large tumor measuring 9.2 x 8.4 cm was observed in the posterior wall of the upper portion of the stomach .
	manualset3
130290	1	405471	5	NULL	NULL	0	NULL	Presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of Not5 and ubiquitinated Rps7A in polysome fractions depends upon the Not4 E3 ligase .
	manualset3
130291	2	405471	5	NULL	NULL	0	NULL	Not5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of Not5 and ubiquitinated Rps7A in polysome fractions depends upon the Not4 E3 ligase .
	manualset3
130292	3	405471	5	NULL	NULL	0	NULL	ubiquitinated Rps7A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of Not5 and ubiquitinated Rps7A in polysome fractions depends upon the Not4 E3 ligase .
	manualset3
130293	4	405471	5	NULL	NULL	0	NULL	polysome fractions	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of Not5 and ubiquitinated Rps7A in polysome fractions depends upon the Not4 E3 ligase .
	manualset3
130294	5	405471	5	NULL	NULL	0	NULL	Not4 E3 ligase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of Not5 and ubiquitinated Rps7A in polysome fractions depends upon the Not4 E3 ligase .
	manualset3
130295	1	405472	5	NULL	NULL	0	NULL	Presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of SOCS1 controls the infection-induced lethal inflammatory disease but impairs the bacterial control .
	manualset3
130296	2	405472	5	NULL	NULL	0	NULL	SOCS1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of SOCS1 controls the infection-induced lethal inflammatory disease but impairs the bacterial control .
	manualset3
130297	3	405472	5	NULL	NULL	0	NULL	infection-induced lethal inflammatory disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of SOCS1 controls the infection-induced lethal inflammatory disease but impairs the bacterial control .
	manualset3
130298	4	405472	5	NULL	NULL	0	NULL	bacterial control	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of SOCS1 controls the infection-induced lethal inflammatory disease but impairs the bacterial control .
	manualset3
130299	1	405473	5	NULL	NULL	0	NULL	Presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of broadly cross-reactive neutralizing antibodies is associated with a lower risk of HIV-1 ( subtype B ) transmission both from mother to child and sexually from male to female .
	manualset3
130300	2	405473	5	NULL	NULL	0	NULL	broadly cross-reactive neutralizing antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of broadly cross-reactive neutralizing antibodies is associated with a lower risk of HIV-1 ( subtype B ) transmission both from mother to child and sexually from male to female .
	manualset3
130301	3	405473	5	NULL	NULL	0	NULL	lower risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of broadly cross-reactive neutralizing antibodies is associated with a lower risk of HIV-1 ( subtype B ) transmission both from mother to child and sexually from male to female .
	manualset3
130302	4	405473	5	NULL	NULL	0	NULL	HIV-1 ( subtype B ) transmission	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of broadly cross-reactive neutralizing antibodies is associated with a lower risk of HIV-1 ( subtype B ) transmission both from mother to child and sexually from male to female .
	manualset3
130303	5	405473	5	NULL	NULL	0	NULL	mother 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of broadly cross-reactive neutralizing antibodies is associated with a lower risk of HIV-1 ( subtype B ) transmission both from mother to child and sexually from male to female .
	manualset3
130304	6	405473	5	NULL	NULL	0	NULL	child 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of broadly cross-reactive neutralizing antibodies is associated with a lower risk of HIV-1 ( subtype B ) transmission both from mother to child and sexually from male to female .
	manualset3
130305	7	405473	5	NULL	NULL	0	NULL	male 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of broadly cross-reactive neutralizing antibodies is associated with a lower risk of HIV-1 ( subtype B ) transmission both from mother to child and sexually from male to female .
	manualset3
130306	8	405473	5	NULL	NULL	0	NULL	female 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of broadly cross-reactive neutralizing antibodies is associated with a lower risk of HIV-1 ( subtype B ) transmission both from mother to child and sexually from male to female .
	manualset3
130307	1	405474	5	NULL	NULL	0	NULL	Presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of poly ( A ) in a flavivirus : significant differences between the 3 ' noncoding regions of the genomic RNAs of tick-borne encephalitis virus strains .
	manualset3
130308	2	405474	5	NULL	NULL	0	NULL	 poly ( A )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of poly ( A ) in a flavivirus : significant differences between the 3 ' noncoding regions of the genomic RNAs of tick-borne encephalitis virus strains .
	manualset3
130309	3	405474	5	NULL	NULL	0	NULL	flavivirus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of poly ( A ) in a flavivirus : significant differences between the 3 ' noncoding regions of the genomic RNAs of tick-borne encephalitis virus strains .
	manualset3
130310	4	405474	5	NULL	NULL	0	NULL	3 ' noncoding regions	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of poly ( A ) in a flavivirus : significant differences between the 3 ' noncoding regions of the genomic RNAs of tick-borne encephalitis virus strains .
	manualset3
130311	5	405474	5	NULL	NULL	0	NULL	genomic RNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of poly ( A ) in a flavivirus : significant differences between the 3 ' noncoding regions of the genomic RNAs of tick-borne encephalitis virus strains .
	manualset3
130312	6	405474	5	NULL	NULL	0	NULL	tick-borne encephalitis virus strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of poly ( A ) in a flavivirus : significant differences between the 3 ' noncoding regions of the genomic RNAs of tick-borne encephalitis virus strains .
	manualset3
130313	1	405475	5	NULL	NULL	0	NULL	Presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of various PLC isozymes in normal human lung tissue was studied from surgical specimens .
	manualset3
130314	2	405475	5	NULL	NULL	0	NULL	PLC isozymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of various PLC isozymes in normal human lung tissue was studied from surgical specimens .
	manualset3
130315	3	405475	5	NULL	NULL	0	NULL	normal human lung tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of various PLC isozymes in normal human lung tissue was studied from surgical specimens .
	manualset3
130316	4	405475	5	NULL	NULL	0	NULL	surgical specimens	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Presence of various PLC isozymes in normal human lung tissue was studied from surgical specimens .
	manualset3
130317	1	405476	5	NULL	NULL	0	NULL	case 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Presented here is a case of first degree A-V block with cannon waves .
	manualset3
130318	2	405476	5	NULL	NULL	0	NULL	first degree A-V block	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Presented here is a case of first degree A-V block with cannon waves .
	manualset3
130319	3	405476	5	NULL	NULL	0	NULL	cannon waves	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Presented here is a case of first degree A-V block with cannon waves .
	manualset3
130320	1	405477	5	NULL	NULL	0	NULL	acetylcholinesterase inhibitors	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Presently , acetylcholinesterase inhibitors are the first-line drugs in the treatment of Alzheimer 's disease ( AD ) .
	manualset3
130321	2	405477	5	NULL	NULL	0	NULL	first-line drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Presently , acetylcholinesterase inhibitors are the first-line drugs in the treatment of Alzheimer 's disease ( AD ) .
	manualset3
130322	3	405477	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Presently , acetylcholinesterase inhibitors are the first-line drugs in the treatment of Alzheimer 's disease ( AD ) .
	manualset3
130323	4	405477	5	NULL	NULL	0	NULL	Alzheimer 's disease ( AD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Presently , acetylcholinesterase inhibitors are the first-line drugs in the treatment of Alzheimer 's disease ( AD ) .
	manualset3
130324	1	405478	5	NULL	NULL	0	NULL	short-chain fatty acids	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Presently , short-chain fatty acids , such as propionate ( Prop ) and butyrate , have been substituted effectively for acetate .
	manualset3
130325	2	405478	5	NULL	NULL	0	NULL	propionate ( Prop )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Presently , short-chain fatty acids , such as propionate ( Prop ) and butyrate , have been substituted effectively for acetate .
	manualset3
130326	3	405478	5	NULL	NULL	0	NULL	butyrate 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Presently , short-chain fatty acids , such as propionate ( Prop ) and butyrate , have been substituted effectively for acetate .
	manualset3
130327	4	405478	5	NULL	NULL	0	NULL	acetate 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Presently , short-chain fatty acids , such as propionate ( Prop ) and butyrate , have been substituted effectively for acetate .
	manualset3
130328	1	405479	5	NULL	NULL	0	NULL	latent profile analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A latent profile analysis identified four neighborhood classes : Black , lower-income ; racially mixed , middle-income ; White , middle-income ; and White , upper-income .
	manualset3
130329	2	405479	5	NULL	NULL	0	NULL	four 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A latent profile analysis identified four neighborhood classes : Black , lower-income ; racially mixed , middle-income ; White , middle-income ; and White , upper-income .
	manualset3
130330	3	405479	5	NULL	NULL	0	NULL	neighborhood classes	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A latent profile analysis identified four neighborhood classes : Black , lower-income ; racially mixed , middle-income ; White , middle-income ; and White , upper-income .
	manualset3
130331	4	405479	5	NULL	NULL	0	NULL	Black 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A latent profile analysis identified four neighborhood classes : Black , lower-income ; racially mixed , middle-income ; White , middle-income ; and White , upper-income .
	manualset3
130332	5	405479	5	NULL	NULL	0	NULL	lower-income	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A latent profile analysis identified four neighborhood classes : Black , lower-income ; racially mixed , middle-income ; White , middle-income ; and White , upper-income .
	manualset3
130333	6	405479	5	NULL	NULL	0	NULL	racially mixed	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A latent profile analysis identified four neighborhood classes : Black , lower-income ; racially mixed , middle-income ; White , middle-income ; and White , upper-income .
	manualset3
130334	7	405479	5	NULL	NULL	0	NULL	middle-income	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A latent profile analysis identified four neighborhood classes : Black , lower-income ; racially mixed , middle-income ; White , middle-income ; and White , upper-income .
	manualset3
130335	8	405479	5	NULL	NULL	0	NULL	White 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A latent profile analysis identified four neighborhood classes : Black , lower-income ; racially mixed , middle-income ; White , middle-income ; and White , upper-income .
	manualset3
130336	9	405479	5	NULL	NULL	0	NULL	middle-income	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A latent profile analysis identified four neighborhood classes : Black , lower-income ; racially mixed , middle-income ; White , middle-income ; and White , upper-income .
	manualset3
130337	10	405479	5	NULL	NULL	0	NULL	White 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A latent profile analysis identified four neighborhood classes : Black , lower-income ; racially mixed , middle-income ; White , middle-income ; and White , upper-income .
	manualset3
130338	11	405479	5	NULL	NULL	0	NULL	upper-income	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A latent profile analysis identified four neighborhood classes : Black , lower-income ; racially mixed , middle-income ; White , middle-income ; and White , upper-income .
	manualset3
130339	1	405480	5	NULL	NULL	0	NULL	10 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Presently at least 10 % of all cases of acute renal failure can be attributed to these antibiotics .
	manualset3
130340	2	405480	5	NULL	NULL	0	NULL	cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Presently at least 10 % of all cases of acute renal failure can be attributed to these antibiotics .
	manualset3
130341	3	405480	5	NULL	NULL	0	NULL	acute renal failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Presently at least 10 % of all cases of acute renal failure can be attributed to these antibiotics .
	manualset3
130342	4	405480	5	NULL	NULL	0	NULL	antibiotics 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Presently at least 10 % of all cases of acute renal failure can be attributed to these antibiotics .
	manualset3
130343	1	405481	5	NULL	NULL	0	NULL	nonsteroidal anti-inflammatory drugs ( NSAIDs )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Presently nonsteroidal anti-inflammatory drugs ( NSAIDs ) which are cyclooxygenase ( COX ) inhibitors are being used for the treatment of inflammatory disorders .
	manualset3
130344	2	405481	5	NULL	NULL	0	NULL	cyclooxygenase ( COX ) inhibitors	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Presently nonsteroidal anti-inflammatory drugs ( NSAIDs ) which are cyclooxygenase ( COX ) inhibitors are being used for the treatment of inflammatory disorders .
	manualset3
130345	3	405481	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Presently nonsteroidal anti-inflammatory drugs ( NSAIDs ) which are cyclooxygenase ( COX ) inhibitors are being used for the treatment of inflammatory disorders .
	manualset3
130346	4	405481	5	NULL	NULL	0	NULL	inflammatory disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Presently nonsteroidal anti-inflammatory drugs ( NSAIDs ) which are cyclooxygenase ( COX ) inhibitors are being used for the treatment of inflammatory disorders .
	manualset3
130347	1	405482	5	NULL	NULL	0	NULL	Pressure-volume curves	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Pressure-volume curves of air - and liquid-filled excised lungs-surface tension in situ .
	manualset3
130348	2	405482	5	NULL	NULL	0	NULL	air - and liquid-filled excised lungs-surface tension	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pressure-volume curves of air - and liquid-filled excised lungs-surface tension in situ .
	manualset3
130349	1	405483	5	NULL	NULL	0	NULL	Pressure breathing therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pressure breathing therapy in chronic pulmonary disease .
	manualset3
130350	2	405483	5	NULL	NULL	0	NULL	chronic pulmonary disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pressure breathing therapy in chronic pulmonary disease .
	manualset3
130351	1	405484	5	NULL	NULL	0	NULL	Pressure 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pressure increases induced constriction with significant changes in ( Ca ( 2 + ) ) ( i ) at high pressures ( 60-100 mmHg ) .
	manualset3
130352	2	405484	5	NULL	NULL	0	NULL	induced constriction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pressure increases induced constriction with significant changes in ( Ca ( 2 + ) ) ( i ) at high pressures ( 60-100 mmHg ) .
	manualset3
130353	3	405484	5	NULL	NULL	0	NULL	( Ca ( 2 + ) )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Pressure increases induced constriction with significant changes in ( Ca ( 2 + ) ) ( i ) at high pressures ( 60-100 mmHg ) .
	manualset3
130354	4	405484	5	NULL	NULL	0	NULL	high pressures ( 60-100 mmHg )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pressure increases induced constriction with significant changes in ( Ca ( 2 + ) ) ( i ) at high pressures ( 60-100 mmHg ) .
	manualset3
130355	1	405485	5	NULL	NULL	0	NULL	Pressure ulcers	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pressure ulcers in pediatric critical care : examining the evidence .
	manualset3
130356	2	405485	5	NULL	NULL	0	NULL	pediatric critical care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pressure ulcers in pediatric critical care : examining the evidence .
	manualset3
130357	3	405485	5	NULL	NULL	0	NULL	evidence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pressure ulcers in pediatric critical care : examining the evidence .
	manualset3
130358	1	405486	5	NULL	NULL	0	NULL	Pressure wire	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Pressure wire , Doppler flow wire and echocontrastomyography ) .
	manualset3
130359	2	405486	5	NULL	NULL	0	NULL	Doppler flow wire	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Pressure wire , Doppler flow wire and echocontrastomyography ) .
	manualset3
130360	3	405486	5	NULL	NULL	0	NULL	echocontrastomyography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pressure wire , Doppler flow wire and echocontrastomyography ) .
	manualset3
130361	1	405487	5	NULL	NULL	NULL	NULL	latissimus dorsi free muscle flap	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A latissimus dorsi free muscle flap was transferred to cover the defect and a split thickness skin graft was placed over the muscle flap .
	manualset3
130362	2	405487	5	NULL	NULL	0	NULL	defect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A latissimus dorsi free muscle flap was transferred to cover the defect and a split thickness skin graft was placed over the muscle flap .
	manualset3
130363	3	405487	5	NULL	NULL	0	NULL	split thickness skin graft	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	A latissimus dorsi free muscle flap was transferred to cover the defect and a split thickness skin graft was placed over the muscle flap .
	manualset3
130364	4	405487	5	NULL	NULL	0	NULL	muscle flap	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	A latissimus dorsi free muscle flap was transferred to cover the defect and a split thickness skin graft was placed over the muscle flap .
	manualset3
130365	1	405488	5	NULL	NULL	0	NULL	Pretreatment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of HUVECs with anti-P - or anti-E-selectin function blocking antibodies significantly reduced both , rolling and subsequent arrest of primary AML cells .
	manualset3
130366	2	405488	5	NULL	NULL	0	NULL	HUVECs 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of HUVECs with anti-P - or anti-E-selectin function blocking antibodies significantly reduced both , rolling and subsequent arrest of primary AML cells .
	manualset3
130367	3	405488	5	NULL	NULL	0	NULL	anti-P -selectin function blocking antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of HUVECs with anti-P - or anti-E-selectin function blocking antibodies significantly reduced both , rolling and subsequent arrest of primary AML cells .
	manualset3
130368	4	405488	5	NULL	NULL	0	NULL	anti-E-selectin function blocking antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of HUVECs with anti-P - or anti-E-selectin function blocking antibodies significantly reduced both , rolling and subsequent arrest of primary AML cells .
	manualset3
130369	5	405488	5	NULL	NULL	0	NULL	rolling and subsequent arrest	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of HUVECs with anti-P - or anti-E-selectin function blocking antibodies significantly reduced both , rolling and subsequent arrest of primary AML cells .
	manualset3
130370	6	405488	5	NULL	NULL	0	NULL	primary AML cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of HUVECs with anti-P - or anti-E-selectin function blocking antibodies significantly reduced both , rolling and subsequent arrest of primary AML cells .
	manualset3
130371	1	405489	5	NULL	NULL	0	NULL	Pretreatment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of cells with methyl-beta-cyclodextrin ( MbetaCD ) , a chemical disrupting caveolae structure , inhibits the translocation of PLC-gamma1 to CM as well as phosphatidylinositol ( PtdIns ) turnover .
	manualset3
130372	2	405489	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of cells with methyl-beta-cyclodextrin ( MbetaCD ) , a chemical disrupting caveolae structure , inhibits the translocation of PLC-gamma1 to CM as well as phosphatidylinositol ( PtdIns ) turnover .
	manualset3
130373	3	405489	5	NULL	NULL	0	NULL	methyl-beta-cyclodextrin ( MbetaCD )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of cells with methyl-beta-cyclodextrin ( MbetaCD ) , a chemical disrupting caveolae structure , inhibits the translocation of PLC-gamma1 to CM as well as phosphatidylinositol ( PtdIns ) turnover .
	manualset3
130374	4	405489	5	NULL	NULL	0	NULL	chemical 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of cells with methyl-beta-cyclodextrin ( MbetaCD ) , a chemical disrupting caveolae structure , inhibits the translocation of PLC-gamma1 to CM as well as phosphatidylinositol ( PtdIns ) turnover .
	manualset3
130375	5	405489	5	NULL	NULL	0	NULL	caveolae structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of cells with methyl-beta-cyclodextrin ( MbetaCD ) , a chemical disrupting caveolae structure , inhibits the translocation of PLC-gamma1 to CM as well as phosphatidylinositol ( PtdIns ) turnover .
	manualset3
130376	6	405489	5	NULL	NULL	0	NULL	translocation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of cells with methyl-beta-cyclodextrin ( MbetaCD ) , a chemical disrupting caveolae structure , inhibits the translocation of PLC-gamma1 to CM as well as phosphatidylinositol ( PtdIns ) turnover .
	manualset3
130377	7	405489	5	NULL	NULL	0	NULL	PLC-gamma1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of cells with methyl-beta-cyclodextrin ( MbetaCD ) , a chemical disrupting caveolae structure , inhibits the translocation of PLC-gamma1 to CM as well as phosphatidylinositol ( PtdIns ) turnover .
	manualset3
130378	8	405489	5	NULL	NULL	0	NULL	CM	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of cells with methyl-beta-cyclodextrin ( MbetaCD ) , a chemical disrupting caveolae structure , inhibits the translocation of PLC-gamma1 to CM as well as phosphatidylinositol ( PtdIns ) turnover .
	manualset3
130379	9	405489	5	NULL	NULL	0	NULL	phosphatidylinositol ( PtdIns ) turnover	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of cells with methyl-beta-cyclodextrin ( MbetaCD ) , a chemical disrupting caveolae structure , inhibits the translocation of PLC-gamma1 to CM as well as phosphatidylinositol ( PtdIns ) turnover .
	manualset3
130380	1	405490	5	NULL	NULL	0	NULL	Pretreatment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of guinea-pigs with CV-3988 , BN 52021 or WEB 2086 at doses inhibiting Paf-induced bronchial hyperresponsiveness , had no significant effect on propranolol or indomethacin-induced bronchial hyperresponsiveness .
	manualset3
130381	2	405490	5	NULL	NULL	0	NULL	guinea-pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of guinea-pigs with CV-3988 , BN 52021 or WEB 2086 at doses inhibiting Paf-induced bronchial hyperresponsiveness , had no significant effect on propranolol or indomethacin-induced bronchial hyperresponsiveness .
	manualset3
130382	3	405490	5	NULL	NULL	0	NULL	CV-3988	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of guinea-pigs with CV-3988 , BN 52021 or WEB 2086 at doses inhibiting Paf-induced bronchial hyperresponsiveness , had no significant effect on propranolol or indomethacin-induced bronchial hyperresponsiveness .
	manualset3
130383	4	405490	5	NULL	NULL	0	NULL	BN 52021	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of guinea-pigs with CV-3988 , BN 52021 or WEB 2086 at doses inhibiting Paf-induced bronchial hyperresponsiveness , had no significant effect on propranolol or indomethacin-induced bronchial hyperresponsiveness .
	manualset3
130384	5	405490	5	NULL	NULL	0	NULL	WEB 2086	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of guinea-pigs with CV-3988 , BN 52021 or WEB 2086 at doses inhibiting Paf-induced bronchial hyperresponsiveness , had no significant effect on propranolol or indomethacin-induced bronchial hyperresponsiveness .
	manualset3
130385	6	405490	5	NULL	NULL	0	NULL	doses 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of guinea-pigs with CV-3988 , BN 52021 or WEB 2086 at doses inhibiting Paf-induced bronchial hyperresponsiveness , had no significant effect on propranolol or indomethacin-induced bronchial hyperresponsiveness .
	manualset3
130386	7	405490	5	NULL	NULL	0	NULL	Paf-induced bronchial hyperresponsiveness	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of guinea-pigs with CV-3988 , BN 52021 or WEB 2086 at doses inhibiting Paf-induced bronchial hyperresponsiveness , had no significant effect on propranolol or indomethacin-induced bronchial hyperresponsiveness .
	manualset3
130387	8	405490	5	NULL	NULL	0	NULL	propranolol or indomethacin-induced bronchial hyperresponsiveness	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of guinea-pigs with CV-3988 , BN 52021 or WEB 2086 at doses inhibiting Paf-induced bronchial hyperresponsiveness , had no significant effect on propranolol or indomethacin-induced bronchial hyperresponsiveness .
	manualset3
130388	1	405491	5	NULL	NULL	0	NULL	Pretreatment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of the cells with the Ah receptor blockers 4 , 7-phenanthroline and alpha-naphthoflavone antagonised the effect of TCDD on 3H-Me-glucose uptake .
	manualset3
130389	2	405491	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of the cells with the Ah receptor blockers 4 , 7-phenanthroline and alpha-naphthoflavone antagonised the effect of TCDD on 3H-Me-glucose uptake .
	manualset3
130390	3	405491	5	NULL	NULL	0	NULL	Ah receptor blockers 4 , 7-phenanthroline 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of the cells with the Ah receptor blockers 4 , 7-phenanthroline and alpha-naphthoflavone antagonised the effect of TCDD on 3H-Me-glucose uptake .
	manualset3
130391	4	405491	5	NULL	NULL	0	NULL	Ah receptor blockers alpha-naphthoflavone 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of the cells with the Ah receptor blockers 4 , 7-phenanthroline and alpha-naphthoflavone antagonised the effect of TCDD on 3H-Me-glucose uptake .
	manualset3
130392	5	405491	5	NULL	NULL	0	NULL	TCDD 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of the cells with the Ah receptor blockers 4 , 7-phenanthroline and alpha-naphthoflavone antagonised the effect of TCDD on 3H-Me-glucose uptake .
	manualset3
130393	6	405491	5	NULL	NULL	0	NULL	3H-Me-glucose uptake	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of the cells with the Ah receptor blockers 4 , 7-phenanthroline and alpha-naphthoflavone antagonised the effect of TCDD on 3H-Me-glucose uptake .
	manualset3
130394	1	405492	5	NULL	NULL	0	NULL	Pretreatment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of the effector cells with interferon-gamma did not change their cytotoxic activity .
	manualset3
130395	2	405492	5	NULL	NULL	0	NULL	effector cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of the effector cells with interferon-gamma did not change their cytotoxic activity .
	manualset3
130396	3	405492	5	NULL	NULL	0	NULL	interferon-gamma	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of the effector cells with interferon-gamma did not change their cytotoxic activity .
	manualset3
130397	4	405492	5	NULL	NULL	0	NULL	cytotoxic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of the effector cells with interferon-gamma did not change their cytotoxic activity .
	manualset3
130398	1	405493	5	NULL	NULL	0	NULL	Pretreatment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of these animals with 2 , 4 , 5 , 2 ' , 4 ' , 5 ' - hexachlorobiphenyl ( HCB ) or 3 , 4 , 3 ' , 4 ' - tetrachlorobiphenyl ( TCB ) protected against benzene toxicity for as long as 7 days , but not after 10 days of repeated dosing .
	manualset3
130399	2	405493	5	NULL	NULL	0	NULL	animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of these animals with 2 , 4 , 5 , 2 ' , 4 ' , 5 ' - hexachlorobiphenyl ( HCB ) or 3 , 4 , 3 ' , 4 ' - tetrachlorobiphenyl ( TCB ) protected against benzene toxicity for as long as 7 days , but not after 10 days of repeated dosing .
	manualset3
130400	3	405493	5	NULL	NULL	0	NULL	2 , 4 , 5 , 2 ' , 4 ' , 5 ' - hexachlorobiphenyl ( HCB ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of these animals with 2 , 4 , 5 , 2 ' , 4 ' , 5 ' - hexachlorobiphenyl ( HCB ) or 3 , 4 , 3 ' , 4 ' - tetrachlorobiphenyl ( TCB ) protected against benzene toxicity for as long as 7 days , but not after 10 days of repeated dosing .
	manualset3
130401	4	405493	5	NULL	NULL	0	NULL	3 , 4 , 3 ' , 4 ' - tetrachlorobiphenyl ( TCB )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of these animals with 2 , 4 , 5 , 2 ' , 4 ' , 5 ' - hexachlorobiphenyl ( HCB ) or 3 , 4 , 3 ' , 4 ' - tetrachlorobiphenyl ( TCB ) protected against benzene toxicity for as long as 7 days , but not after 10 days of repeated dosing .
	manualset3
130402	5	405493	5	NULL	NULL	0	NULL	benzene toxicity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of these animals with 2 , 4 , 5 , 2 ' , 4 ' , 5 ' - hexachlorobiphenyl ( HCB ) or 3 , 4 , 3 ' , 4 ' - tetrachlorobiphenyl ( TCB ) protected against benzene toxicity for as long as 7 days , but not after 10 days of repeated dosing .
	manualset3
130403	6	405493	5	NULL	NULL	0	NULL	7 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of these animals with 2 , 4 , 5 , 2 ' , 4 ' , 5 ' - hexachlorobiphenyl ( HCB ) or 3 , 4 , 3 ' , 4 ' - tetrachlorobiphenyl ( TCB ) protected against benzene toxicity for as long as 7 days , but not after 10 days of repeated dosing .
	manualset3
130404	7	405493	5	NULL	NULL	0	NULL	10 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of these animals with 2 , 4 , 5 , 2 ' , 4 ' , 5 ' - hexachlorobiphenyl ( HCB ) or 3 , 4 , 3 ' , 4 ' - tetrachlorobiphenyl ( TCB ) protected against benzene toxicity for as long as 7 days , but not after 10 days of repeated dosing .
	manualset3
130405	1	405494	5	NULL	NULL	0	NULL	Pretreatment surgical staging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment surgical staging of patients with cervical carcinoma : the case for lymph node debulking .
	manualset3
130406	2	405494	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment surgical staging of patients with cervical carcinoma : the case for lymph node debulking .
	manualset3
130407	3	405494	5	NULL	NULL	0	NULL	cervical carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment surgical staging of patients with cervical carcinoma : the case for lymph node debulking .
	manualset3
130408	4	405494	5	NULL	NULL	0	NULL	case 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment surgical staging of patients with cervical carcinoma : the case for lymph node debulking .
	manualset3
130409	5	405494	5	NULL	NULL	0	NULL	lymph node debulking 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment surgical staging of patients with cervical carcinoma : the case for lymph node debulking .
	manualset3
130410	1	405495	5	NULL	NULL	0	NULL	Pretreatment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with 0.2 microM ecdysone for 48 h prior to exposure to H2O2 , increased viability to 77 % of controls .
	manualset3
130411	2	405495	5	NULL	NULL	0	NULL	 0.2 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with 0.2 microM ecdysone for 48 h prior to exposure to H2O2 , increased viability to 77 % of controls .
	manualset3
130412	3	405495	5	NULL	NULL	0	NULL	ecdysone 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with 0.2 microM ecdysone for 48 h prior to exposure to H2O2 , increased viability to 77 % of controls .
	manualset3
130413	4	405495	5	NULL	NULL	0	NULL	48 h 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with 0.2 microM ecdysone for 48 h prior to exposure to H2O2 , increased viability to 77 % of controls .
	manualset3
130414	5	405495	5	NULL	NULL	0	NULL	exposure 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with 0.2 microM ecdysone for 48 h prior to exposure to H2O2 , increased viability to 77 % of controls .
	manualset3
130415	6	405495	5	NULL	NULL	0	NULL	H2O2 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with 0.2 microM ecdysone for 48 h prior to exposure to H2O2 , increased viability to 77 % of controls .
	manualset3
130416	7	405495	5	NULL	NULL	0	NULL	viability 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with 0.2 microM ecdysone for 48 h prior to exposure to H2O2 , increased viability to 77 % of controls .
	manualset3
130417	8	405495	5	NULL	NULL	0	NULL	77 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with 0.2 microM ecdysone for 48 h prior to exposure to H2O2 , increased viability to 77 % of controls .
	manualset3
130418	9	405495	5	NULL	NULL	0	NULL	controls 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with 0.2 microM ecdysone for 48 h prior to exposure to H2O2 , increased viability to 77 % of controls .
	manualset3
130419	1	405496	5	NULL	NULL	0	NULL	Pretreatment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with 6-hydroxydopamine , a neurotoxin selective for sympathetic postganglionic nerve terminals , had no effect on release evoked by 1.5 % formalin , but significantly reduced adenosine release during the late phase of release induced by 5 % formalin .
	manualset3
130420	2	405496	5	NULL	NULL	0	NULL	6-hydroxydopamine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with 6-hydroxydopamine , a neurotoxin selective for sympathetic postganglionic nerve terminals , had no effect on release evoked by 1.5 % formalin , but significantly reduced adenosine release during the late phase of release induced by 5 % formalin .
	manualset3
130421	3	405496	5	NULL	NULL	0	NULL	neurotoxin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with 6-hydroxydopamine , a neurotoxin selective for sympathetic postganglionic nerve terminals , had no effect on release evoked by 1.5 % formalin , but significantly reduced adenosine release during the late phase of release induced by 5 % formalin .
	manualset3
130422	4	405496	5	NULL	NULL	0	NULL	sympathetic postganglionic nerve terminals	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with 6-hydroxydopamine , a neurotoxin selective for sympathetic postganglionic nerve terminals , had no effect on release evoked by 1.5 % formalin , but significantly reduced adenosine release during the late phase of release induced by 5 % formalin .
	manualset3
130423	5	405496	5	NULL	NULL	0	NULL	1.5 % formalin	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with 6-hydroxydopamine , a neurotoxin selective for sympathetic postganglionic nerve terminals , had no effect on release evoked by 1.5 % formalin , but significantly reduced adenosine release during the late phase of release induced by 5 % formalin .
	manualset3
130424	6	405496	5	NULL	NULL	NULL	NULL	adenosine 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pretreatment with 6-hydroxydopamine , a neurotoxin selective for sympathetic postganglionic nerve terminals , had no effect on release evoked by 1.5 % formalin , but significantly reduced adenosine release during the late phase of release induced by 5 % formalin .
	manualset3
130425	7	405496	5	NULL	NULL	0	NULL	 late phase of release	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with 6-hydroxydopamine , a neurotoxin selective for sympathetic postganglionic nerve terminals , had no effect on release evoked by 1.5 % formalin , but significantly reduced adenosine release during the late phase of release induced by 5 % formalin .
	manualset3
130426	8	405496	5	NULL	NULL	0	NULL	5 % formalin	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with 6-hydroxydopamine , a neurotoxin selective for sympathetic postganglionic nerve terminals , had no effect on release evoked by 1.5 % formalin , but significantly reduced adenosine release during the late phase of release induced by 5 % formalin .
	manualset3
130427	1	405497	5	NULL	NULL	0	NULL	Pretreatment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with LH or PGE2 desensitized the cells to further hormone stimulation , while the forskolin response was unaffected .
	manualset3
130428	2	405497	5	NULL	NULL	0	NULL	LH 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with LH or PGE2 desensitized the cells to further hormone stimulation , while the forskolin response was unaffected .
	manualset3
130429	3	405497	5	NULL	NULL	0	NULL	PGE2	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with LH or PGE2 desensitized the cells to further hormone stimulation , while the forskolin response was unaffected .
	manualset3
130430	4	405497	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with LH or PGE2 desensitized the cells to further hormone stimulation , while the forskolin response was unaffected .
	manualset3
130431	5	405497	5	NULL	NULL	0	NULL	hormone stimulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with LH or PGE2 desensitized the cells to further hormone stimulation , while the forskolin response was unaffected .
	manualset3
130432	6	405497	5	NULL	NULL	0	NULL	forskolin response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with LH or PGE2 desensitized the cells to further hormone stimulation , while the forskolin response was unaffected .
	manualset3
130433	1	405498	5	NULL	NULL	0	NULL	leaflet 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A leaflet including advices for C-V prevention was distributed to the whole S community in 1976 .
	manualset3
130434	2	405498	5	NULL	NULL	0	NULL	advices 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A leaflet including advices for C-V prevention was distributed to the whole S community in 1976 .
	manualset3
130435	3	405498	5	NULL	NULL	0	NULL	C-V prevention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A leaflet including advices for C-V prevention was distributed to the whole S community in 1976 .
	manualset3
130436	4	405498	5	NULL	NULL	0	NULL	S community	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A leaflet including advices for C-V prevention was distributed to the whole S community in 1976 .
	manualset3
130437	5	405498	5	NULL	NULL	0	NULL	1976	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	A leaflet including advices for C-V prevention was distributed to the whole S community in 1976 .
	manualset3
130438	1	405499	5	NULL	NULL	0	NULL	Pretreatment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with a sublethal concentration of pisatin induced the amoebae to acquire resistance to both these effects .
	manualset3
130439	2	405499	5	NULL	NULL	0	NULL	sublethal concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with a sublethal concentration of pisatin induced the amoebae to acquire resistance to both these effects .
	manualset3
130440	3	405499	5	NULL	NULL	0	NULL	pisatin 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with a sublethal concentration of pisatin induced the amoebae to acquire resistance to both these effects .
	manualset3
130441	4	405499	5	NULL	NULL	0	NULL	amoebae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with a sublethal concentration of pisatin induced the amoebae to acquire resistance to both these effects .
	manualset3
130442	5	405499	5	NULL	NULL	0	NULL	resistance 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with a sublethal concentration of pisatin induced the amoebae to acquire resistance to both these effects .
	manualset3
130443	1	405500	5	NULL	NULL	0	NULL	Pretreatment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with dexamethasone inhibited APNEA-induced degranulation of mast cells in the thymus and slightly , yet significantly , reduced degranulation induced by compound 48/80 .
	manualset3
130444	2	405500	5	NULL	NULL	0	NULL	dexamethasone 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with dexamethasone inhibited APNEA-induced degranulation of mast cells in the thymus and slightly , yet significantly , reduced degranulation induced by compound 48/80 .
	manualset3
130445	3	405500	5	NULL	NULL	NULL	NULL	APNEA-induced degranulation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pretreatment with dexamethasone inhibited APNEA-induced degranulation of mast cells in the thymus and slightly , yet significantly , reduced degranulation induced by compound 48/80 .
	manualset3
130446	4	405500	5	NULL	NULL	0	NULL	mast cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with dexamethasone inhibited APNEA-induced degranulation of mast cells in the thymus and slightly , yet significantly , reduced degranulation induced by compound 48/80 .
	manualset3
130447	5	405500	5	NULL	NULL	0	NULL	thymus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with dexamethasone inhibited APNEA-induced degranulation of mast cells in the thymus and slightly , yet significantly , reduced degranulation induced by compound 48/80 .
	manualset3
130448	6	405500	5	NULL	NULL	NULL	NULL	degranulation 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pretreatment with dexamethasone inhibited APNEA-induced degranulation of mast cells in the thymus and slightly , yet significantly , reduced degranulation induced by compound 48/80 .
	manualset3
130449	7	405500	5	NULL	NULL	0	NULL	compound 48/80	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with dexamethasone inhibited APNEA-induced degranulation of mast cells in the thymus and slightly , yet significantly , reduced degranulation induced by compound 48/80 .
	manualset3
131057	1	405501	5	NULL	NULL	0	NULL	Pretreatment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with haloperidol reduces ( 123 ) I-FP-CIT binding to the dopamine transporter in the rat striatum : an in vivo imaging study with a dedicated small-animal SPECT camera .
	manualset3
131058	2	405501	5	NULL	NULL	0	NULL	haloperidol 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with haloperidol reduces ( 123 ) I-FP-CIT binding to the dopamine transporter in the rat striatum : an in vivo imaging study with a dedicated small-animal SPECT camera .
	manualset3
131059	3	405501	5	NULL	NULL	0	NULL	( 123 ) I-FP-CIT 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with haloperidol reduces ( 123 ) I-FP-CIT binding to the dopamine transporter in the rat striatum : an in vivo imaging study with a dedicated small-animal SPECT camera .
	manualset3
131060	4	405501	5	NULL	NULL	0	NULL	dopamine transporter	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with haloperidol reduces ( 123 ) I-FP-CIT binding to the dopamine transporter in the rat striatum : an in vivo imaging study with a dedicated small-animal SPECT camera .
	manualset3
131061	5	405501	5	NULL	NULL	0	NULL	rat striatum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with haloperidol reduces ( 123 ) I-FP-CIT binding to the dopamine transporter in the rat striatum : an in vivo imaging study with a dedicated small-animal SPECT camera .
	manualset3
131062	6	405501	5	NULL	NULL	0	NULL	in vivo imaging study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with haloperidol reduces ( 123 ) I-FP-CIT binding to the dopamine transporter in the rat striatum : an in vivo imaging study with a dedicated small-animal SPECT camera .
	manualset3
131063	7	405501	5	NULL	NULL	0	NULL	small-animal SPECT camera	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with haloperidol reduces ( 123 ) I-FP-CIT binding to the dopamine transporter in the rat striatum : an in vivo imaging study with a dedicated small-animal SPECT camera .
	manualset3
131064	1	405502	5	NULL	NULL	0	NULL	Prevalence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence and intensity of helminth infections ( egg counts/g stool ) of Ascaris lumbricoides , Trichuris trichiura and hookworms significantly fell in the 2 groups receiving anthelmintic treatment and there were some reductions in the 2 groups not receiving anthelminthic treatment .
	manualset3
131065	2	405502	5	NULL	NULL	0	NULL	intensity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence and intensity of helminth infections ( egg counts/g stool ) of Ascaris lumbricoides , Trichuris trichiura and hookworms significantly fell in the 2 groups receiving anthelmintic treatment and there were some reductions in the 2 groups not receiving anthelminthic treatment .
	manualset3
131066	3	405502	5	NULL	NULL	0	NULL	helminth infections 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence and intensity of helminth infections ( egg counts/g stool ) of Ascaris lumbricoides , Trichuris trichiura and hookworms significantly fell in the 2 groups receiving anthelmintic treatment and there were some reductions in the 2 groups not receiving anthelminthic treatment .
	manualset3
131067	4	405502	5	NULL	NULL	0	NULL	 egg counts/g stool	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence and intensity of helminth infections ( egg counts/g stool ) of Ascaris lumbricoides , Trichuris trichiura and hookworms significantly fell in the 2 groups receiving anthelmintic treatment and there were some reductions in the 2 groups not receiving anthelminthic treatment .
	manualset3
131068	5	405502	5	NULL	NULL	0	NULL	Ascaris lumbricoides	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence and intensity of helminth infections ( egg counts/g stool ) of Ascaris lumbricoides , Trichuris trichiura and hookworms significantly fell in the 2 groups receiving anthelmintic treatment and there were some reductions in the 2 groups not receiving anthelminthic treatment .
	manualset3
131069	6	405502	5	NULL	NULL	0	NULL	Trichuris trichiura	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence and intensity of helminth infections ( egg counts/g stool ) of Ascaris lumbricoides , Trichuris trichiura and hookworms significantly fell in the 2 groups receiving anthelmintic treatment and there were some reductions in the 2 groups not receiving anthelminthic treatment .
	manualset3
131070	7	405502	5	NULL	NULL	0	NULL	hookworms 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence and intensity of helminth infections ( egg counts/g stool ) of Ascaris lumbricoides , Trichuris trichiura and hookworms significantly fell in the 2 groups receiving anthelmintic treatment and there were some reductions in the 2 groups not receiving anthelminthic treatment .
	manualset3
131071	8	405502	5	NULL	NULL	0	NULL	2 groups	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence and intensity of helminth infections ( egg counts/g stool ) of Ascaris lumbricoides , Trichuris trichiura and hookworms significantly fell in the 2 groups receiving anthelmintic treatment and there were some reductions in the 2 groups not receiving anthelminthic treatment .
	manualset3
131072	9	405502	5	NULL	NULL	0	NULL	anthelmintic treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence and intensity of helminth infections ( egg counts/g stool ) of Ascaris lumbricoides , Trichuris trichiura and hookworms significantly fell in the 2 groups receiving anthelmintic treatment and there were some reductions in the 2 groups not receiving anthelminthic treatment .
	manualset3
131073	10	405502	5	NULL	NULL	0	NULL	reductions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence and intensity of helminth infections ( egg counts/g stool ) of Ascaris lumbricoides , Trichuris trichiura and hookworms significantly fell in the 2 groups receiving anthelmintic treatment and there were some reductions in the 2 groups not receiving anthelminthic treatment .
	manualset3
131074	11	405502	5	NULL	NULL	0	NULL	2 groups	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence and intensity of helminth infections ( egg counts/g stool ) of Ascaris lumbricoides , Trichuris trichiura and hookworms significantly fell in the 2 groups receiving anthelmintic treatment and there were some reductions in the 2 groups not receiving anthelminthic treatment .
	manualset3
131075	12	405502	5	NULL	NULL	0	NULL	anthelminthic treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence and intensity of helminth infections ( egg counts/g stool ) of Ascaris lumbricoides , Trichuris trichiura and hookworms significantly fell in the 2 groups receiving anthelmintic treatment and there were some reductions in the 2 groups not receiving anthelminthic treatment .
	manualset3
131076	1	405503	5	NULL	NULL	0	NULL	Prevalence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of BHV-2 in the herd was determined by using BHV-2 SNT at 7 occasions during a period of 15 months .
	manualset3
131077	2	405503	5	NULL	NULL	0	NULL	 BHV-2	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of BHV-2 in the herd was determined by using BHV-2 SNT at 7 occasions during a period of 15 months .
	manualset3
131078	3	405503	5	NULL	NULL	0	NULL	herd 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of BHV-2 in the herd was determined by using BHV-2 SNT at 7 occasions during a period of 15 months .
	manualset3
131079	4	405503	5	NULL	NULL	0	NULL	BHV-2 SNT	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of BHV-2 in the herd was determined by using BHV-2 SNT at 7 occasions during a period of 15 months .
	manualset3
131080	5	405503	5	NULL	NULL	0	NULL	7 occasions	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of BHV-2 in the herd was determined by using BHV-2 SNT at 7 occasions during a period of 15 months .
	manualset3
131081	6	405503	5	NULL	NULL	0	NULL	period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of BHV-2 in the herd was determined by using BHV-2 SNT at 7 occasions during a period of 15 months .
	manualset3
131082	7	405503	5	NULL	NULL	0	NULL	15 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of BHV-2 in the herd was determined by using BHV-2 SNT at 7 occasions during a period of 15 months .
	manualset3
131083	1	405504	5	NULL	NULL	0	NULL	Prevalence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of CPV and CDV varied significantly among years .
	manualset3
131084	2	405504	5	NULL	NULL	0	NULL	CPV 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of CPV and CDV varied significantly among years .
	manualset3
131085	3	405504	5	NULL	NULL	0	NULL	CDV 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of CPV and CDV varied significantly among years .
	manualset3
131086	4	405504	5	NULL	NULL	0	NULL	years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of CPV and CDV varied significantly among years .
	manualset3
131087	1	405505	5	NULL	NULL	0	NULL	leptospiral whole cell lysate	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A leptospiral whole cell lysate from each serovar was used as the antigen to react with IgG and IgM in the sera from four patients with a positive MAT .
	manualset3
131088	2	405505	5	NULL	NULL	0	NULL	serovar 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A leptospiral whole cell lysate from each serovar was used as the antigen to react with IgG and IgM in the sera from four patients with a positive MAT .
	manualset3
131089	3	405505	5	NULL	NULL	0	NULL	antigen 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A leptospiral whole cell lysate from each serovar was used as the antigen to react with IgG and IgM in the sera from four patients with a positive MAT .
	manualset3
131090	4	405505	5	NULL	NULL	0	NULL	IgG	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A leptospiral whole cell lysate from each serovar was used as the antigen to react with IgG and IgM in the sera from four patients with a positive MAT .
	manualset3
131091	5	405505	5	NULL	NULL	0	NULL	IgM 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A leptospiral whole cell lysate from each serovar was used as the antigen to react with IgG and IgM in the sera from four patients with a positive MAT .
	manualset3
131092	6	405505	5	NULL	NULL	0	NULL	sera 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A leptospiral whole cell lysate from each serovar was used as the antigen to react with IgG and IgM in the sera from four patients with a positive MAT .
	manualset3
131093	7	405505	5	NULL	NULL	0	NULL	four 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A leptospiral whole cell lysate from each serovar was used as the antigen to react with IgG and IgM in the sera from four patients with a positive MAT .
	manualset3
131094	8	405505	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A leptospiral whole cell lysate from each serovar was used as the antigen to react with IgG and IgM in the sera from four patients with a positive MAT .
	manualset3
131095	9	405505	5	NULL	NULL	0	NULL	positive MAT	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A leptospiral whole cell lysate from each serovar was used as the antigen to react with IgG and IgM in the sera from four patients with a positive MAT .
	manualset3
131096	1	405506	5	NULL	NULL	0	NULL	Prevalence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of Mycoplasma pneumoniae in subjectively healthy individuals .
	manualset3
131097	2	405506	5	NULL	NULL	0	NULL	Mycoplasma pneumoniae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of Mycoplasma pneumoniae in subjectively healthy individuals .
	manualset3
131098	3	405506	5	NULL	NULL	0	NULL	healthy individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of Mycoplasma pneumoniae in subjectively healthy individuals .
	manualset3
131099	1	405507	5	NULL	NULL	0	NULL	Prevalence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of bovine immunodeficiency virus infection in cattle in Great Britain .
	manualset3
131100	2	405507	5	NULL	NULL	0	NULL	bovine immunodeficiency virus infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of bovine immunodeficiency virus infection in cattle in Great Britain .
	manualset3
131101	3	405507	5	NULL	NULL	0	NULL	cattle 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of bovine immunodeficiency virus infection in cattle in Great Britain .
	manualset3
131102	4	405507	5	NULL	NULL	0	NULL	Great Britain	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of bovine immunodeficiency virus infection in cattle in Great Britain .
	manualset3
131103	1	405508	5	NULL	NULL	0	NULL	Prevalence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of cholelithiasis in men and women ingesting a serum-cholesterol-lowering diet .
	manualset3
131104	2	405508	5	NULL	NULL	0	NULL	cholelithiasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of cholelithiasis in men and women ingesting a serum-cholesterol-lowering diet .
	manualset3
131105	3	405508	5	NULL	NULL	0	NULL	men 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of cholelithiasis in men and women ingesting a serum-cholesterol-lowering diet .
	manualset3
131106	4	405508	5	NULL	NULL	0	NULL	women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of cholelithiasis in men and women ingesting a serum-cholesterol-lowering diet .
	manualset3
131107	5	405508	5	NULL	NULL	0	NULL	serum-cholesterol-lowering diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of cholelithiasis in men and women ingesting a serum-cholesterol-lowering diet .
	manualset3
131108	1	405509	5	NULL	NULL	0	NULL	Prevalence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of exercise-induced bronchospasm in a cohort of varsity college athletes .
	manualset3
131109	2	405509	5	NULL	NULL	0	NULL	exercise-induced bronchospasm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of exercise-induced bronchospasm in a cohort of varsity college athletes .
	manualset3
131110	3	405509	5	NULL	NULL	0	NULL	cohort of varsity college athletes	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of exercise-induced bronchospasm in a cohort of varsity college athletes .
	manualset3
131111	1	405510	5	NULL	NULL	0	NULL	Prevalence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of female genital cutting in Upper Egypt : 6 years after enforcement of prohibition law .
	manualset3
131112	2	405510	5	NULL	NULL	0	NULL	female genital cutting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of female genital cutting in Upper Egypt : 6 years after enforcement of prohibition law .
	manualset3
131113	3	405510	5	NULL	NULL	0	NULL	Upper Egypt	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of female genital cutting in Upper Egypt : 6 years after enforcement of prohibition law .
	manualset3
131114	4	405510	5	NULL	NULL	0	NULL	6 year	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of female genital cutting in Upper Egypt : 6 years after enforcement of prohibition law .
	manualset3
131115	5	405510	5	NULL	NULL	0	NULL	enforcement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of female genital cutting in Upper Egypt : 6 years after enforcement of prohibition law .
	manualset3
131116	6	405510	5	NULL	NULL	0	NULL	prohibition law	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of female genital cutting in Upper Egypt : 6 years after enforcement of prohibition law .
	manualset3
131117	1	405511	5	NULL	NULL	0	NULL	Prevalence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of human papillomavirus in mobile tongue cancer with particular reference to young patients .
	manualset3
131118	2	405511	5	NULL	NULL	0	NULL	human papillomavirus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of human papillomavirus in mobile tongue cancer with particular reference to young patients .
	manualset3
131119	3	405511	5	NULL	NULL	0	NULL	mobile tongue cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of human papillomavirus in mobile tongue cancer with particular reference to young patients .
	manualset3
131120	4	405511	5	NULL	NULL	0	NULL	young patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of human papillomavirus in mobile tongue cancer with particular reference to young patients .
	manualset3
131121	1	405512	5	NULL	NULL	0	NULL	Prevalence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of retinopathy of prematurity in Latin America .
	manualset3
131122	2	405512	5	NULL	NULL	0	NULL	retinopathy 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of retinopathy of prematurity in Latin America .
	manualset3
131123	3	405512	5	NULL	NULL	0	NULL	Latin America	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of retinopathy of prematurity in Latin America .
	manualset3
134860	4	405512	5	NULL	NULL	0	NULL	prematurity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of retinopathy of prematurity in Latin America .
	manualset3
131124	1	405513	5	NULL	NULL	NULL	NULL	Prevalence 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Prevalence of virulence determinants in Staphylococcus epidermidis from ICU patients in Kampala , Uganda .
	manualset3
131125	2	405513	5	NULL	NULL	0	NULL	virulence determinants	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of virulence determinants in Staphylococcus epidermidis from ICU patients in Kampala , Uganda .
	manualset3
131126	3	405513	5	NULL	NULL	0	NULL	Staphylococcus epidermidis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of virulence determinants in Staphylococcus epidermidis from ICU patients in Kampala , Uganda .
	manualset3
131127	4	405513	5	NULL	NULL	0	NULL	ICU patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of virulence determinants in Staphylococcus epidermidis from ICU patients in Kampala , Uganda .
	manualset3
131128	5	405513	5	NULL	NULL	0	NULL	Kampala , Uganda	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of virulence determinants in Staphylococcus epidermidis from ICU patients in Kampala , Uganda .
	manualset3
131129	1	405514	5	NULL	NULL	0	NULL	Prevalence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of viruses in colonies of laboratory rodents .
	manualset3
131130	2	405514	5	NULL	NULL	0	NULL	viruses 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of viruses in colonies of laboratory rodents .
	manualset3
131131	3	405514	5	NULL	NULL	0	NULL	colonies of laboratory rodents	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of viruses in colonies of laboratory rodents .
	manualset3
131132	1	405515	5	NULL	NULL	0	NULL	A2A agonist , N6 - ( 2 - ( 3 , 5-dimethyoxyphenyl ) -2 - ( 2-methylphenyl ) - ethyl ) adenosine	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A less potent A2A agonist , N6 - ( 2 - ( 3 , 5-dimethyoxyphenyl ) -2 - ( 2-methylphenyl ) - ethyl ) adenosine ( 1 mg/kg ) , provided only partial protection against kainate .
	manualset3
131133	2	405515	5	NULL	NULL	0	NULL	1 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A less potent A2A agonist , N6 - ( 2 - ( 3 , 5-dimethyoxyphenyl ) -2 - ( 2-methylphenyl ) - ethyl ) adenosine ( 1 mg/kg ) , provided only partial protection against kainate .
	manualset3
131134	3	405515	5	NULL	NULL	0	NULL	partial protection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A less potent A2A agonist , N6 - ( 2 - ( 3 , 5-dimethyoxyphenyl ) -2 - ( 2-methylphenyl ) - ethyl ) adenosine ( 1 mg/kg ) , provided only partial protection against kainate .
	manualset3
131135	4	405515	5	NULL	NULL	0	NULL	kainate 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A less potent A2A agonist , N6 - ( 2 - ( 3 , 5-dimethyoxyphenyl ) -2 - ( 2-methylphenyl ) - ethyl ) adenosine ( 1 mg/kg ) , provided only partial protection against kainate .
	manualset3
131136	1	405516	5	NULL	NULL	0	NULL	Prevention 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of coronary heart disease through cholesterol reduction .
	manualset3
131137	2	405516	5	NULL	NULL	0	NULL	coronary heart disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of coronary heart disease through cholesterol reduction .
	manualset3
131138	3	405516	5	NULL	NULL	0	NULL	cholesterol reduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of coronary heart disease through cholesterol reduction .
	manualset3
131139	1	405517	5	NULL	NULL	0	NULL	Prevention 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of diabetes and diabetes-related complications through treatment and disease self-management is paramount in changing this deadly and costly course and demands continued innovation in health programs and services and new partnerships among health professionals .
	manualset3
131140	2	405517	5	NULL	NULL	0	NULL	diabetes 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of diabetes and diabetes-related complications through treatment and disease self-management is paramount in changing this deadly and costly course and demands continued innovation in health programs and services and new partnerships among health professionals .
	manualset3
131141	3	405517	5	NULL	NULL	0	NULL	diabetes-related complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of diabetes and diabetes-related complications through treatment and disease self-management is paramount in changing this deadly and costly course and demands continued innovation in health programs and services and new partnerships among health professionals .
	manualset3
131142	4	405517	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of diabetes and diabetes-related complications through treatment and disease self-management is paramount in changing this deadly and costly course and demands continued innovation in health programs and services and new partnerships among health professionals .
	manualset3
131143	5	405517	5	NULL	NULL	0	NULL	disease self-management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of diabetes and diabetes-related complications through treatment and disease self-management is paramount in changing this deadly and costly course and demands continued innovation in health programs and services and new partnerships among health professionals .
	manualset3
131144	6	405517	5	NULL	NULL	0	NULL	deadly and costly course	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of diabetes and diabetes-related complications through treatment and disease self-management is paramount in changing this deadly and costly course and demands continued innovation in health programs and services and new partnerships among health professionals .
	manualset3
131145	7	405517	5	NULL	NULL	0	NULL	innovation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of diabetes and diabetes-related complications through treatment and disease self-management is paramount in changing this deadly and costly course and demands continued innovation in health programs and services and new partnerships among health professionals .
	manualset3
131146	8	405517	5	NULL	NULL	0	NULL	health programs 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of diabetes and diabetes-related complications through treatment and disease self-management is paramount in changing this deadly and costly course and demands continued innovation in health programs and services and new partnerships among health professionals .
	manualset3
131147	9	405517	5	NULL	NULL	0	NULL	services	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of diabetes and diabetes-related complications through treatment and disease self-management is paramount in changing this deadly and costly course and demands continued innovation in health programs and services and new partnerships among health professionals .
	manualset3
131148	10	405517	5	NULL	NULL	0	NULL	partnerships 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of diabetes and diabetes-related complications through treatment and disease self-management is paramount in changing this deadly and costly course and demands continued innovation in health programs and services and new partnerships among health professionals .
	manualset3
131149	11	405517	5	NULL	NULL	0	NULL	health professionals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of diabetes and diabetes-related complications through treatment and disease self-management is paramount in changing this deadly and costly course and demands continued innovation in health programs and services and new partnerships among health professionals .
	manualset3
131150	1	405518	5	NULL	NULL	0	NULL	Prevention 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of hip fractures in long-term care : relevance of community-derived data .
	manualset3
131151	2	405518	5	NULL	NULL	0	NULL	hip fractures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of hip fractures in long-term care : relevance of community-derived data .
	manualset3
131152	3	405518	5	NULL	NULL	0	NULL	long-term care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of hip fractures in long-term care : relevance of community-derived data .
	manualset3
131153	4	405518	5	NULL	NULL	0	NULL	relevance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of hip fractures in long-term care : relevance of community-derived data .
	manualset3
131154	5	405518	5	NULL	NULL	0	NULL	community-derived data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of hip fractures in long-term care : relevance of community-derived data .
	manualset3
131155	1	405519	5	NULL	NULL	0	NULL	Prevention 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of maternal HIV transmission .
	manualset3
131156	2	405519	5	NULL	NULL	0	NULL	maternal HIV transmission	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of maternal HIV transmission .
	manualset3
131157	1	405520	5	NULL	NULL	0	NULL	Prevention 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of poultry-borne salmonellosis by irradiation : costs and benefits in Scotland .
	manualset3
131158	2	405520	5	NULL	NULL	0	NULL	poultry-borne salmonellosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of poultry-borne salmonellosis by irradiation : costs and benefits in Scotland .
	manualset3
131159	3	405520	5	NULL	NULL	0	NULL	irradiation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of poultry-borne salmonellosis by irradiation : costs and benefits in Scotland .
	manualset3
131160	4	405520	5	NULL	NULL	0	NULL	costs 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of poultry-borne salmonellosis by irradiation : costs and benefits in Scotland .
	manualset3
131161	5	405520	5	NULL	NULL	0	NULL	benefits 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of poultry-borne salmonellosis by irradiation : costs and benefits in Scotland .
	manualset3
131162	6	405520	5	NULL	NULL	0	NULL	Scotland 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of poultry-borne salmonellosis by irradiation : costs and benefits in Scotland .
	manualset3
131163	1	405521	5	NULL	NULL	0	NULL	Prevention 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of the crankshaft phenomenon .
	manualset3
131164	2	405521	5	NULL	NULL	0	NULL	crankshaft phenomenon	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of the crankshaft phenomenon .
	manualset3
131165	1	405522	5	NULL	NULL	0	NULL	Prevention 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of toxicity was suggested in the second evaluation period in which none of the patients , having therapy altered by the notification , developed toxicity versus 13 of the 40 other patients who developed a rise in serum creatinine concentration or a reduction in hearing acuity .
	manualset3
131166	2	405522	5	NULL	NULL	0	NULL	toxicity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of toxicity was suggested in the second evaluation period in which none of the patients , having therapy altered by the notification , developed toxicity versus 13 of the 40 other patients who developed a rise in serum creatinine concentration or a reduction in hearing acuity .
	manualset3
131167	3	405522	5	NULL	NULL	0	NULL	second evaluation period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of toxicity was suggested in the second evaluation period in which none of the patients , having therapy altered by the notification , developed toxicity versus 13 of the 40 other patients who developed a rise in serum creatinine concentration or a reduction in hearing acuity .
	manualset3
131168	4	405522	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of toxicity was suggested in the second evaluation period in which none of the patients , having therapy altered by the notification , developed toxicity versus 13 of the 40 other patients who developed a rise in serum creatinine concentration or a reduction in hearing acuity .
	manualset3
131169	5	405522	5	NULL	NULL	0	NULL	therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of toxicity was suggested in the second evaluation period in which none of the patients , having therapy altered by the notification , developed toxicity versus 13 of the 40 other patients who developed a rise in serum creatinine concentration or a reduction in hearing acuity .
	manualset3
131170	6	405522	5	NULL	NULL	0	NULL	notification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of toxicity was suggested in the second evaluation period in which none of the patients , having therapy altered by the notification , developed toxicity versus 13 of the 40 other patients who developed a rise in serum creatinine concentration or a reduction in hearing acuity .
	manualset3
131171	7	405522	5	NULL	NULL	0	NULL	toxicity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of toxicity was suggested in the second evaluation period in which none of the patients , having therapy altered by the notification , developed toxicity versus 13 of the 40 other patients who developed a rise in serum creatinine concentration or a reduction in hearing acuity .
	manualset3
131172	8	405522	5	NULL	NULL	0	NULL	13 of the 40 other patients	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of toxicity was suggested in the second evaluation period in which none of the patients , having therapy altered by the notification , developed toxicity versus 13 of the 40 other patients who developed a rise in serum creatinine concentration or a reduction in hearing acuity .
	manualset3
131173	9	405522	5	NULL	NULL	0	NULL	serum creatinine concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of toxicity was suggested in the second evaluation period in which none of the patients , having therapy altered by the notification , developed toxicity versus 13 of the 40 other patients who developed a rise in serum creatinine concentration or a reduction in hearing acuity .
	manualset3
131174	10	405522	5	NULL	NULL	0	NULL	reduction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of toxicity was suggested in the second evaluation period in which none of the patients , having therapy altered by the notification , developed toxicity versus 13 of the 40 other patients who developed a rise in serum creatinine concentration or a reduction in hearing acuity .
	manualset3
131175	11	405522	5	NULL	NULL	0	NULL	hearing acuity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of toxicity was suggested in the second evaluation period in which none of the patients , having therapy altered by the notification , developed toxicity versus 13 of the 40 other patients who developed a rise in serum creatinine concentration or a reduction in hearing acuity .
	manualset3
131176	1	405523	5	NULL	NULL	0	NULL	lethal factor	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A lethal factor in the blood of rabbits following occlusion of the superior mesentric artery .
	manualset3
131177	2	405523	5	NULL	NULL	0	NULL	blood 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	A lethal factor in the blood of rabbits following occlusion of the superior mesentric artery .
	manualset3
131178	3	405523	5	NULL	NULL	0	NULL	rabbits 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A lethal factor in the blood of rabbits following occlusion of the superior mesentric artery .
	manualset3
131179	4	405523	5	NULL	NULL	0	NULL	occlusion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A lethal factor in the blood of rabbits following occlusion of the superior mesentric artery .
	manualset3
131180	5	405523	5	NULL	NULL	0	NULL	superior mesentric artery 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A lethal factor in the blood of rabbits following occlusion of the superior mesentric artery .
	manualset3
131181	1	405524	5	NULL	NULL	0	NULL	EPS proteomic studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous EPS proteomic studies of activated sludge revealed several problems , like the interference of other EPS molecules in protein analysis .
	manualset3
131182	2	405524	5	NULL	NULL	0	NULL	activated sludge	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous EPS proteomic studies of activated sludge revealed several problems , like the interference of other EPS molecules in protein analysis .
	manualset3
131183	3	405524	5	NULL	NULL	0	NULL	problems 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous EPS proteomic studies of activated sludge revealed several problems , like the interference of other EPS molecules in protein analysis .
	manualset3
131184	4	405524	5	NULL	NULL	0	NULL	interference 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous EPS proteomic studies of activated sludge revealed several problems , like the interference of other EPS molecules in protein analysis .
	manualset3
131185	5	405524	5	NULL	NULL	0	NULL	 EPS molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous EPS proteomic studies of activated sludge revealed several problems , like the interference of other EPS molecules in protein analysis .
	manualset3
131186	6	405524	5	NULL	NULL	0	NULL	protein analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous EPS proteomic studies of activated sludge revealed several problems , like the interference of other EPS molecules in protein analysis .
	manualset3
131187	1	405525	5	NULL	NULL	0	NULL	chronic blockade	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous chronic blockade of NMDA receptors intensifies morphine dependence in rats .
	manualset3
131188	2	405525	5	NULL	NULL	0	NULL	NMDA receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous chronic blockade of NMDA receptors intensifies morphine dependence in rats .
	manualset3
131189	3	405525	5	NULL	NULL	0	NULL	morphine dependence	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous chronic blockade of NMDA receptors intensifies morphine dependence in rats .
	manualset3
131190	4	405525	5	NULL	NULL	0	NULL	rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous chronic blockade of NMDA receptors intensifies morphine dependence in rats .
	manualset3
131191	1	405526	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous data have shown that HEPES , a taurine structural analog , inhibits the uptake of taurine by cultured cells differently , depending on its addition either to the culture medium or to the Krebs-Ringer buffer used for cell incubation during taurine uptake measurements ( Lleu and Rebel , J Neurosci Res 23 : 78-86 , 1989 ) .
	manualset3
131192	2	405526	5	NULL	NULL	0	NULL	HEPES , a taurine structural analog	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous data have shown that HEPES , a taurine structural analog , inhibits the uptake of taurine by cultured cells differently , depending on its addition either to the culture medium or to the Krebs-Ringer buffer used for cell incubation during taurine uptake measurements ( Lleu and Rebel , J Neurosci Res 23 : 78-86 , 1989 ) .
	manualset3
131193	3	405526	5	NULL	NULL	0	NULL	uptake 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous data have shown that HEPES , a taurine structural analog , inhibits the uptake of taurine by cultured cells differently , depending on its addition either to the culture medium or to the Krebs-Ringer buffer used for cell incubation during taurine uptake measurements ( Lleu and Rebel , J Neurosci Res 23 : 78-86 , 1989 ) .
	manualset3
131194	4	405526	5	NULL	NULL	0	NULL	taurine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous data have shown that HEPES , a taurine structural analog , inhibits the uptake of taurine by cultured cells differently , depending on its addition either to the culture medium or to the Krebs-Ringer buffer used for cell incubation during taurine uptake measurements ( Lleu and Rebel , J Neurosci Res 23 : 78-86 , 1989 ) .
	manualset3
131195	5	405526	5	NULL	NULL	0	NULL	cultured cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous data have shown that HEPES , a taurine structural analog , inhibits the uptake of taurine by cultured cells differently , depending on its addition either to the culture medium or to the Krebs-Ringer buffer used for cell incubation during taurine uptake measurements ( Lleu and Rebel , J Neurosci Res 23 : 78-86 , 1989 ) .
	manualset3
131196	6	405526	5	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous data have shown that HEPES , a taurine structural analog , inhibits the uptake of taurine by cultured cells differently , depending on its addition either to the culture medium or to the Krebs-Ringer buffer used for cell incubation during taurine uptake measurements ( Lleu and Rebel , J Neurosci Res 23 : 78-86 , 1989 ) .
	manualset3
131197	7	405526	5	NULL	NULL	0	NULL	culture medium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous data have shown that HEPES , a taurine structural analog , inhibits the uptake of taurine by cultured cells differently , depending on its addition either to the culture medium or to the Krebs-Ringer buffer used for cell incubation during taurine uptake measurements ( Lleu and Rebel , J Neurosci Res 23 : 78-86 , 1989 ) .
	manualset3
131198	8	405526	5	NULL	NULL	0	NULL	Krebs-Ringer buffer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous data have shown that HEPES , a taurine structural analog , inhibits the uptake of taurine by cultured cells differently , depending on its addition either to the culture medium or to the Krebs-Ringer buffer used for cell incubation during taurine uptake measurements ( Lleu and Rebel , J Neurosci Res 23 : 78-86 , 1989 ) .
	manualset3
131199	9	405526	5	NULL	NULL	0	NULL	cell incubation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous data have shown that HEPES , a taurine structural analog , inhibits the uptake of taurine by cultured cells differently , depending on its addition either to the culture medium or to the Krebs-Ringer buffer used for cell incubation during taurine uptake measurements ( Lleu and Rebel , J Neurosci Res 23 : 78-86 , 1989 ) .
	manualset3
131200	10	405526	5	NULL	NULL	0	NULL	taurine uptake measurements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous data have shown that HEPES , a taurine structural analog , inhibits the uptake of taurine by cultured cells differently , depending on its addition either to the culture medium or to the Krebs-Ringer buffer used for cell incubation during taurine uptake measurements ( Lleu and Rebel , J Neurosci Res 23 : 78-86 , 1989 ) .
	manualset3
131201	11	405526	5	NULL	NULL	0	NULL	Lleu and Rebel , J Neurosci Res 23 : 78-86 , 1989	Citation												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous data have shown that HEPES , a taurine structural analog , inhibits the uptake of taurine by cultured cells differently , depending on its addition either to the culture medium or to the Krebs-Ringer buffer used for cell incubation during taurine uptake measurements ( Lleu and Rebel , J Neurosci Res 23 : 78-86 , 1989 ) .
	manualset3
131202	1	405527	5	NULL	NULL	0	NULL	examinations 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous examinations of breast cancer and survival in Hawai'i 's 5 major ethnic groups have found that Native Hawaiian women have the highest breast cancer mortality rates .
	manualset3
131203	2	405527	5	NULL	NULL	0	NULL	breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous examinations of breast cancer and survival in Hawai'i 's 5 major ethnic groups have found that Native Hawaiian women have the highest breast cancer mortality rates .
	manualset3
131204	3	405527	5	NULL	NULL	0	NULL	survival 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous examinations of breast cancer and survival in Hawai'i 's 5 major ethnic groups have found that Native Hawaiian women have the highest breast cancer mortality rates .
	manualset3
131205	4	405527	5	NULL	NULL	0	NULL	Hawai'i	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous examinations of breast cancer and survival in Hawai'i 's 5 major ethnic groups have found that Native Hawaiian women have the highest breast cancer mortality rates .
	manualset3
131206	5	405527	5	NULL	NULL	0	NULL	5 major ethnic groups	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous examinations of breast cancer and survival in Hawai'i 's 5 major ethnic groups have found that Native Hawaiian women have the highest breast cancer mortality rates .
	manualset3
131207	6	405527	5	NULL	NULL	0	NULL	Native Hawaiian women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous examinations of breast cancer and survival in Hawai'i 's 5 major ethnic groups have found that Native Hawaiian women have the highest breast cancer mortality rates .
	manualset3
131208	7	405527	5	NULL	NULL	0	NULL	breast cancer mortality rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous examinations of breast cancer and survival in Hawai'i 's 5 major ethnic groups have found that Native Hawaiian women have the highest breast cancer mortality rates .
	manualset3
131209	1	405528	5	NULL	NULL	0	NULL	experimental studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous experimental studies of collaborative competition analyzed cases in which target sites for pairs of cooperating TFs were contained within the same side of the nucleosome .
	manualset3
131210	2	405528	5	NULL	NULL	0	NULL	collaborative competition analyzed cases	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous experimental studies of collaborative competition analyzed cases in which target sites for pairs of cooperating TFs were contained within the same side of the nucleosome .
	manualset3
131211	3	405528	5	NULL	NULL	0	NULL	target sites	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous experimental studies of collaborative competition analyzed cases in which target sites for pairs of cooperating TFs were contained within the same side of the nucleosome .
	manualset3
131212	4	405528	5	NULL	NULL	0	NULL	pairs of cooperating TFs 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous experimental studies of collaborative competition analyzed cases in which target sites for pairs of cooperating TFs were contained within the same side of the nucleosome .
	manualset3
131213	5	405528	5	NULL	NULL	0	NULL	same side	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous experimental studies of collaborative competition analyzed cases in which target sites for pairs of cooperating TFs were contained within the same side of the nucleosome .
	manualset3
131214	6	405528	5	NULL	NULL	0	NULL	nucleosome 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous experimental studies of collaborative competition analyzed cases in which target sites for pairs of cooperating TFs were contained within the same side of the nucleosome .
	manualset3
131215	1	405529	5	NULL	NULL	0	NULL	microarray studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous microarray studies identified individual genes as candidates for alcohol phenotypes , but efforts to generate an integrated view of molecular and cellular changes underlying alcohol addiction are lacking .
	manualset3
131216	2	405529	5	NULL	NULL	0	NULL	individual genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous microarray studies identified individual genes as candidates for alcohol phenotypes , but efforts to generate an integrated view of molecular and cellular changes underlying alcohol addiction are lacking .
	manualset3
131217	3	405529	5	NULL	NULL	0	NULL	candidates 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous microarray studies identified individual genes as candidates for alcohol phenotypes , but efforts to generate an integrated view of molecular and cellular changes underlying alcohol addiction are lacking .
	manualset3
131218	4	405529	5	NULL	NULL	NULL	NULL	alcohol phenotypes	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Previous microarray studies identified individual genes as candidates for alcohol phenotypes , but efforts to generate an integrated view of molecular and cellular changes underlying alcohol addiction are lacking .
	manualset3
131219	5	405529	5	NULL	NULL	0	NULL	integrated view 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous microarray studies identified individual genes as candidates for alcohol phenotypes , but efforts to generate an integrated view of molecular and cellular changes underlying alcohol addiction are lacking .
	manualset3
131220	6	405529	5	NULL	NULL	0	NULL	molecular changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous microarray studies identified individual genes as candidates for alcohol phenotypes , but efforts to generate an integrated view of molecular and cellular changes underlying alcohol addiction are lacking .
	manualset3
131221	7	405529	5	NULL	NULL	0	NULL	cellular changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous microarray studies identified individual genes as candidates for alcohol phenotypes , but efforts to generate an integrated view of molecular and cellular changes underlying alcohol addiction are lacking .
	manualset3
131222	8	405529	5	NULL	NULL	0	NULL	alcohol addiction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous microarray studies identified individual genes as candidates for alcohol phenotypes , but efforts to generate an integrated view of molecular and cellular changes underlying alcohol addiction are lacking .
	manualset3
131223	1	405530	5	NULL	NULL	0	NULL	publications 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous publications have reported two conflicting patterns describing the relationship between income and suicide in Sweden ; positive and negative .
	manualset3
131224	2	405530	5	NULL	NULL	0	NULL	conflicting patterns	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous publications have reported two conflicting patterns describing the relationship between income and suicide in Sweden ; positive and negative .
	manualset3
131225	3	405530	5	NULL	NULL	0	NULL	relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous publications have reported two conflicting patterns describing the relationship between income and suicide in Sweden ; positive and negative .
	manualset3
131226	4	405530	5	NULL	NULL	0	NULL	income 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous publications have reported two conflicting patterns describing the relationship between income and suicide in Sweden ; positive and negative .
	manualset3
131227	5	405530	5	NULL	NULL	0	NULL	suicide 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous publications have reported two conflicting patterns describing the relationship between income and suicide in Sweden ; positive and negative .
	manualset3
131228	6	405530	5	NULL	NULL	0	NULL	Sweden 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous publications have reported two conflicting patterns describing the relationship between income and suicide in Sweden ; positive and negative .
	manualset3
126589	1	405531	13	NULL	NULL	0	NULL	letter	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A letter to Ms. Fujiwara in Colombia ) .
	manualset3
126590	2	405531	13	NULL	NULL	0	NULL	Ms. Fujiwara	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A letter to Ms. Fujiwara in Colombia ) .
	manualset3
126591	3	405531	13	NULL	NULL	0	NULL	Colombia	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A letter to Ms. Fujiwara in Colombia ) .
	manualset3
126592	1	405532	13	NULL	NULL	0	NULL	reports	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous reports from our laboratory have indicated that the elongation step is specially affected by aging as a consequence of alterations in elongation factor-2 ( eEF-2 ) .
	manualset3
126593	2	405532	13	NULL	NULL	0	NULL	laboratory	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous reports from our laboratory have indicated that the elongation step is specially affected by aging as a consequence of alterations in elongation factor-2 ( eEF-2 ) .
	manualset3
126594	3	405532	13	NULL	NULL	0	NULL	elongation step 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous reports from our laboratory have indicated that the elongation step is specially affected by aging as a consequence of alterations in elongation factor-2 ( eEF-2 ) .
	manualset3
126595	4	405532	13	NULL	NULL	0	NULL	consequence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous reports from our laboratory have indicated that the elongation step is specially affected by aging as a consequence of alterations in elongation factor-2 ( eEF-2 ) .
	manualset3
126596	5	405532	13	NULL	NULL	0	NULL	alterations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous reports from our laboratory have indicated that the elongation step is specially affected by aging as a consequence of alterations in elongation factor-2 ( eEF-2 ) .
	manualset3
126597	6	405532	13	NULL	NULL	0	NULL	elongation factor-2 ( eEF-2 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous reports from our laboratory have indicated that the elongation step is specially affected by aging as a consequence of alterations in elongation factor-2 ( eEF-2 ) .
	manualset3
128811	7	405532	13	NULL	NULL	0	NULL	aging 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous reports from our laboratory have indicated that the elongation step is specially affected by aging as a consequence of alterations in elongation factor-2 ( eEF-2 ) .
	manualset3
126598	1	405533	13	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous research has shown that in lifting an object , grip force rises with the increase in gravitational load force as the hand takes the weight and that in moving an object , grip force is adjusted to meet movement-induced inertial load force .
	manualset3
126599	2	405533	13	NULL	NULL	0	NULL	object	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous research has shown that in lifting an object , grip force rises with the increase in gravitational load force as the hand takes the weight and that in moving an object , grip force is adjusted to meet movement-induced inertial load force .
	manualset3
126600	3	405533	13	NULL	NULL	0	NULL	 grip force	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous research has shown that in lifting an object , grip force rises with the increase in gravitational load force as the hand takes the weight and that in moving an object , grip force is adjusted to meet movement-induced inertial load force .
	manualset3
126601	4	405533	13	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous research has shown that in lifting an object , grip force rises with the increase in gravitational load force as the hand takes the weight and that in moving an object , grip force is adjusted to meet movement-induced inertial load force .
	manualset3
126602	5	405533	13	NULL	NULL	0	NULL	gravitational load force	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous research has shown that in lifting an object , grip force rises with the increase in gravitational load force as the hand takes the weight and that in moving an object , grip force is adjusted to meet movement-induced inertial load force .
	manualset3
126603	6	405533	13	NULL	NULL	0	NULL	hand	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous research has shown that in lifting an object , grip force rises with the increase in gravitational load force as the hand takes the weight and that in moving an object , grip force is adjusted to meet movement-induced inertial load force .
	manualset3
126604	7	405533	13	NULL	NULL	0	NULL	weight	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous research has shown that in lifting an object , grip force rises with the increase in gravitational load force as the hand takes the weight and that in moving an object , grip force is adjusted to meet movement-induced inertial load force .
	manualset3
126605	8	405533	13	NULL	NULL	0	NULL	object	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous research has shown that in lifting an object , grip force rises with the increase in gravitational load force as the hand takes the weight and that in moving an object , grip force is adjusted to meet movement-induced inertial load force .
	manualset3
126606	9	405533	13	NULL	NULL	0	NULL	grip force	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous research has shown that in lifting an object , grip force rises with the increase in gravitational load force as the hand takes the weight and that in moving an object , grip force is adjusted to meet movement-induced inertial load force .
	manualset3
126607	10	405533	13	NULL	NULL	0	NULL	inertial load force 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous research has shown that in lifting an object , grip force rises with the increase in gravitational load force as the hand takes the weight and that in moving an object , grip force is adjusted to meet movement-induced inertial load force .
	manualset3
126608	1	405534	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous results using paired-pulse transcranial magnetic stimulation ( TMS ) have suggested that the excitability of transcallosal ( TC ) connections between the hand areas of the two motor cortices is modulated by intracortical inhibitory circuits in the same way as corticospinal tract ( CTS ) projections to spinal motoneurons .
	manualset3
126609	2	405534	13	NULL	NULL	0	NULL	paired-pulse transcranial magnetic stimulation ( TMS )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous results using paired-pulse transcranial magnetic stimulation ( TMS ) have suggested that the excitability of transcallosal ( TC ) connections between the hand areas of the two motor cortices is modulated by intracortical inhibitory circuits in the same way as corticospinal tract ( CTS ) projections to spinal motoneurons .
	manualset3
126610	3	405534	13	NULL	NULL	0	NULL	excitability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous results using paired-pulse transcranial magnetic stimulation ( TMS ) have suggested that the excitability of transcallosal ( TC ) connections between the hand areas of the two motor cortices is modulated by intracortical inhibitory circuits in the same way as corticospinal tract ( CTS ) projections to spinal motoneurons .
	manualset3
126611	4	405534	13	NULL	NULL	0	NULL	transcallosal ( TC ) connections 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous results using paired-pulse transcranial magnetic stimulation ( TMS ) have suggested that the excitability of transcallosal ( TC ) connections between the hand areas of the two motor cortices is modulated by intracortical inhibitory circuits in the same way as corticospinal tract ( CTS ) projections to spinal motoneurons .
	manualset3
126612	5	405534	13	NULL	NULL	0	NULL	hand areas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous results using paired-pulse transcranial magnetic stimulation ( TMS ) have suggested that the excitability of transcallosal ( TC ) connections between the hand areas of the two motor cortices is modulated by intracortical inhibitory circuits in the same way as corticospinal tract ( CTS ) projections to spinal motoneurons .
	manualset3
126613	6	405534	13	NULL	NULL	0	NULL	two motor cortices 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous results using paired-pulse transcranial magnetic stimulation ( TMS ) have suggested that the excitability of transcallosal ( TC ) connections between the hand areas of the two motor cortices is modulated by intracortical inhibitory circuits in the same way as corticospinal tract ( CTS ) projections to spinal motoneurons .
	manualset3
126614	7	405534	13	NULL	NULL	0	NULL	intracortical inhibitory circuits 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous results using paired-pulse transcranial magnetic stimulation ( TMS ) have suggested that the excitability of transcallosal ( TC ) connections between the hand areas of the two motor cortices is modulated by intracortical inhibitory circuits in the same way as corticospinal tract ( CTS ) projections to spinal motoneurons .
	manualset3
126615	8	405534	13	NULL	NULL	0	NULL	corticospinal tract ( CTS ) projections	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous results using paired-pulse transcranial magnetic stimulation ( TMS ) have suggested that the excitability of transcallosal ( TC ) connections between the hand areas of the two motor cortices is modulated by intracortical inhibitory circuits in the same way as corticospinal tract ( CTS ) projections to spinal motoneurons .
	manualset3
126616	9	405534	13	NULL	NULL	0	NULL	spinal motoneurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous results using paired-pulse transcranial magnetic stimulation ( TMS ) have suggested that the excitability of transcallosal ( TC ) connections between the hand areas of the two motor cortices is modulated by intracortical inhibitory circuits in the same way as corticospinal tract ( CTS ) projections to spinal motoneurons .
	manualset3
126617	1	405535	13	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies established that following simultaneous injection of 125I-labeled homologous very low density lipoproteins ( VLDL ) and 131I-labeled homologous low density lipoproteins ( LDL ) into miniature pigs , a large proportion of LDL apolipoprotein B ( apoB ) was synthesized directly , independent of VLDL or intermediate density lipoprotein ( IDL ) apoB catabolism .
	manualset3
126618	2	405535	13	NULL	NULL	0	NULL	injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies established that following simultaneous injection of 125I-labeled homologous very low density lipoproteins ( VLDL ) and 131I-labeled homologous low density lipoproteins ( LDL ) into miniature pigs , a large proportion of LDL apolipoprotein B ( apoB ) was synthesized directly , independent of VLDL or intermediate density lipoprotein ( IDL ) apoB catabolism .
	manualset3
126619	3	405535	13	NULL	NULL	0	NULL	125I-labeled homologous very low density lipoproteins ( VLDL ) 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies established that following simultaneous injection of 125I-labeled homologous very low density lipoproteins ( VLDL ) and 131I-labeled homologous low density lipoproteins ( LDL ) into miniature pigs , a large proportion of LDL apolipoprotein B ( apoB ) was synthesized directly , independent of VLDL or intermediate density lipoprotein ( IDL ) apoB catabolism .
	manualset3
126620	4	405535	13	NULL	NULL	0	NULL	131I-labeled homologous low density lipoproteins ( LDL )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies established that following simultaneous injection of 125I-labeled homologous very low density lipoproteins ( VLDL ) and 131I-labeled homologous low density lipoproteins ( LDL ) into miniature pigs , a large proportion of LDL apolipoprotein B ( apoB ) was synthesized directly , independent of VLDL or intermediate density lipoprotein ( IDL ) apoB catabolism .
	manualset3
126621	5	405535	13	NULL	NULL	0	NULL	miniature pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies established that following simultaneous injection of 125I-labeled homologous very low density lipoproteins ( VLDL ) and 131I-labeled homologous low density lipoproteins ( LDL ) into miniature pigs , a large proportion of LDL apolipoprotein B ( apoB ) was synthesized directly , independent of VLDL or intermediate density lipoprotein ( IDL ) apoB catabolism .
	manualset3
126622	6	405535	13	NULL	NULL	0	NULL	large proportion	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies established that following simultaneous injection of 125I-labeled homologous very low density lipoproteins ( VLDL ) and 131I-labeled homologous low density lipoproteins ( LDL ) into miniature pigs , a large proportion of LDL apolipoprotein B ( apoB ) was synthesized directly , independent of VLDL or intermediate density lipoprotein ( IDL ) apoB catabolism .
	manualset3
126623	7	405535	13	NULL	NULL	0	NULL	LDL apolipoprotein B ( apoB ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies established that following simultaneous injection of 125I-labeled homologous very low density lipoproteins ( VLDL ) and 131I-labeled homologous low density lipoproteins ( LDL ) into miniature pigs , a large proportion of LDL apolipoprotein B ( apoB ) was synthesized directly , independent of VLDL or intermediate density lipoprotein ( IDL ) apoB catabolism .
	manualset3
126624	8	405535	13	NULL	NULL	NULL	NULL	VLDL catabolism	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Previous studies established that following simultaneous injection of 125I-labeled homologous very low density lipoproteins ( VLDL ) and 131I-labeled homologous low density lipoproteins ( LDL ) into miniature pigs , a large proportion of LDL apolipoprotein B ( apoB ) was synthesized directly , independent of VLDL or intermediate density lipoprotein ( IDL ) apoB catabolism .
	manualset3
126625	9	405535	13	NULL	NULL	0	NULL	intermediate density lipoprotein ( IDL ) apoB catabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies established that following simultaneous injection of 125I-labeled homologous very low density lipoproteins ( VLDL ) and 131I-labeled homologous low density lipoproteins ( LDL ) into miniature pigs , a large proportion of LDL apolipoprotein B ( apoB ) was synthesized directly , independent of VLDL or intermediate density lipoprotein ( IDL ) apoB catabolism .
	manualset3
126626	1	405536	13	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies have demonstrated that SHP-1 plays a role in determining signal strength from the TCR .
	manualset3
126627	2	405536	13	NULL	NULL	0	NULL	SHP-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies have demonstrated that SHP-1 plays a role in determining signal strength from the TCR .
	manualset3
126628	3	405536	13	NULL	NULL	0	NULL	role 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies have demonstrated that SHP-1 plays a role in determining signal strength from the TCR .
	manualset3
126629	4	405536	13	NULL	NULL	0	NULL	signal strength	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies have demonstrated that SHP-1 plays a role in determining signal strength from the TCR .
	manualset3
126630	5	405536	13	NULL	NULL	0	NULL	TCR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies have demonstrated that SHP-1 plays a role in determining signal strength from the TCR .
	manualset3
126631	1	405537	13	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies have shown that food deprivation , which occurs naturally in the life cycle of many species of fish , results in cessation of growth and catabolism of stored energy reserves , including lipids .
	manualset3
126632	2	405537	13	NULL	NULL	0	NULL	food	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies have shown that food deprivation , which occurs naturally in the life cycle of many species of fish , results in cessation of growth and catabolism of stored energy reserves , including lipids .
	manualset3
126633	3	405537	13	NULL	NULL	0	NULL	deprivation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies have shown that food deprivation , which occurs naturally in the life cycle of many species of fish , results in cessation of growth and catabolism of stored energy reserves , including lipids .
	manualset3
126634	4	405537	13	NULL	NULL	0	NULL	life cycle 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies have shown that food deprivation , which occurs naturally in the life cycle of many species of fish , results in cessation of growth and catabolism of stored energy reserves , including lipids .
	manualset3
126635	5	405537	13	NULL	NULL	0	NULL	species of fish	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies have shown that food deprivation , which occurs naturally in the life cycle of many species of fish , results in cessation of growth and catabolism of stored energy reserves , including lipids .
	manualset3
126637	7	405537	13	NULL	NULL	NULL	NULL	cessation of growth	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Previous studies have shown that food deprivation , which occurs naturally in the life cycle of many species of fish , results in cessation of growth and catabolism of stored energy reserves , including lipids .
	manualset3
126639	9	405537	13	NULL	NULL	0	NULL	catabolism of stored energy reserves	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies have shown that food deprivation , which occurs naturally in the life cycle of many species of fish , results in cessation of growth and catabolism of stored energy reserves , including lipids .
	manualset3
126640	10	405537	13	NULL	NULL	0	NULL	lipids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies have shown that food deprivation , which occurs naturally in the life cycle of many species of fish , results in cessation of growth and catabolism of stored energy reserves , including lipids .
	manualset3
126641	1	405538	13	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies have suggested major effects on mononuclear cell cytokine production and T cell migration , but results have been inconsistent .
	manualset3
126642	2	405538	13	NULL	NULL	0	NULL	major effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies have suggested major effects on mononuclear cell cytokine production and T cell migration , but results have been inconsistent .
	manualset3
126643	3	405538	13	NULL	NULL	0	NULL	mononuclear cell cytokine production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies have suggested major effects on mononuclear cell cytokine production and T cell migration , but results have been inconsistent .
	manualset3
126644	4	405538	13	NULL	NULL	0	NULL	T cell migration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies have suggested major effects on mononuclear cell cytokine production and T cell migration , but results have been inconsistent .
	manualset3
126645	5	405538	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies have suggested major effects on mononuclear cell cytokine production and T cell migration , but results have been inconsistent .
	manualset3
126646	1	405539	13	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies with an asparagus PR10 gene ( AoPR1 ) promoter in heterologous plants suggested that the AoPR10-GUS transgene was responsive to oxidative signals/stresses .
	manualset3
126647	2	405539	13	NULL	NULL	0	NULL	asparagus PR10 gene ( AoPR1 ) promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies with an asparagus PR10 gene ( AoPR1 ) promoter in heterologous plants suggested that the AoPR10-GUS transgene was responsive to oxidative signals/stresses .
	manualset3
126648	3	405539	13	NULL	NULL	0	NULL	heterologous plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies with an asparagus PR10 gene ( AoPR1 ) promoter in heterologous plants suggested that the AoPR10-GUS transgene was responsive to oxidative signals/stresses .
	manualset3
126649	4	405539	13	NULL	NULL	0	NULL	AoPR10-GUS transgene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies with an asparagus PR10 gene ( AoPR1 ) promoter in heterologous plants suggested that the AoPR10-GUS transgene was responsive to oxidative signals/stresses .
	manualset3
126650	5	405539	13	NULL	NULL	0	NULL	oxidative signals/stresses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies with an asparagus PR10 gene ( AoPR1 ) promoter in heterologous plants suggested that the AoPR10-GUS transgene was responsive to oxidative signals/stresses .
	manualset3
126651	1	405540	13	NULL	NULL	0	NULL	work	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous work from this laboratory showed that generation of memory CD8 T cells by different immunization routes correlates with control of tumors growing in distinct sites .
	manualset3
126652	2	405540	13	NULL	NULL	0	NULL	laboratory 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous work from this laboratory showed that generation of memory CD8 T cells by different immunization routes correlates with control of tumors growing in distinct sites .
	manualset3
126653	3	405540	13	NULL	NULL	0	NULL	generation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous work from this laboratory showed that generation of memory CD8 T cells by different immunization routes correlates with control of tumors growing in distinct sites .
	manualset3
126654	4	405540	13	NULL	NULL	0	NULL	memory CD8 T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous work from this laboratory showed that generation of memory CD8 T cells by different immunization routes correlates with control of tumors growing in distinct sites .
	manualset3
126655	5	405540	13	NULL	NULL	0	NULL	immunization routes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous work from this laboratory showed that generation of memory CD8 T cells by different immunization routes correlates with control of tumors growing in distinct sites .
	manualset3
126656	6	405540	13	NULL	NULL	0	NULL	control 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous work from this laboratory showed that generation of memory CD8 T cells by different immunization routes correlates with control of tumors growing in distinct sites .
	manualset3
126657	7	405540	13	NULL	NULL	0	NULL	tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous work from this laboratory showed that generation of memory CD8 T cells by different immunization routes correlates with control of tumors growing in distinct sites .
	manualset3
126658	8	405540	13	NULL	NULL	0	NULL	distinct sites 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous work from this laboratory showed that generation of memory CD8 T cells by different immunization routes correlates with control of tumors growing in distinct sites .
	manualset3
126659	1	405541	13	NULL	NULL	0	NULL	work	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous work has indicated that systemic capsaicin administration causes permanent neuronal degeneration in neonatal rats , but evidence that capsaicin has a similar effect in adults is equivocal and incomplete .
	manualset3
126660	2	405541	13	NULL	NULL	0	NULL	systemic capsaicin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous work has indicated that systemic capsaicin administration causes permanent neuronal degeneration in neonatal rats , but evidence that capsaicin has a similar effect in adults is equivocal and incomplete .
	manualset3
126661	3	405541	13	NULL	NULL	0	NULL	administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous work has indicated that systemic capsaicin administration causes permanent neuronal degeneration in neonatal rats , but evidence that capsaicin has a similar effect in adults is equivocal and incomplete .
	manualset3
126663	5	405541	13	NULL	NULL	0	NULL	neuronal degeneration 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous work has indicated that systemic capsaicin administration causes permanent neuronal degeneration in neonatal rats , but evidence that capsaicin has a similar effect in adults is equivocal and incomplete .
	manualset3
126664	6	405541	13	NULL	NULL	0	NULL	neonatal rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous work has indicated that systemic capsaicin administration causes permanent neuronal degeneration in neonatal rats , but evidence that capsaicin has a similar effect in adults is equivocal and incomplete .
	manualset3
126665	7	405541	13	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous work has indicated that systemic capsaicin administration causes permanent neuronal degeneration in neonatal rats , but evidence that capsaicin has a similar effect in adults is equivocal and incomplete .
	manualset3
126666	8	405541	13	NULL	NULL	0	NULL	capsaicin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous work has indicated that systemic capsaicin administration causes permanent neuronal degeneration in neonatal rats , but evidence that capsaicin has a similar effect in adults is equivocal and incomplete .
	manualset3
126667	9	405541	13	NULL	NULL	0	NULL	similar effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous work has indicated that systemic capsaicin administration causes permanent neuronal degeneration in neonatal rats , but evidence that capsaicin has a similar effect in adults is equivocal and incomplete .
	manualset3
126668	10	405541	13	NULL	NULL	0	NULL	adults	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous work has indicated that systemic capsaicin administration causes permanent neuronal degeneration in neonatal rats , but evidence that capsaicin has a similar effect in adults is equivocal and incomplete .
	manualset3
126669	1	405542	13	NULL	NULL	0	NULL	life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A life free of drug reps. Come into obstetrics .
	manualset3
126670	2	405542	13	NULL	NULL	0	NULL	drug reps	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A life free of drug reps. Come into obstetrics .
	manualset3
126671	3	405542	13	NULL	NULL	0	NULL	obstetrics	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A life free of drug reps. Come into obstetrics .
	manualset3
126672	1	405543	13	NULL	NULL	0	NULL	work	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous work has shown that several products emerging from lipid peroxidation ( e.g. lipid hydroperoxides , lysophospholipids , oxidized cholesterol ) are able to reduce NO production in macrophages .
	manualset3
126673	2	405543	13	NULL	NULL	0	NULL	products	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous work has shown that several products emerging from lipid peroxidation ( e.g. lipid hydroperoxides , lysophospholipids , oxidized cholesterol ) are able to reduce NO production in macrophages .
	manualset3
126674	3	405543	13	NULL	NULL	0	NULL	lipid peroxidation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous work has shown that several products emerging from lipid peroxidation ( e.g. lipid hydroperoxides , lysophospholipids , oxidized cholesterol ) are able to reduce NO production in macrophages .
	manualset3
126675	4	405543	13	NULL	NULL	NULL	NULL	lipid hydroperoxides	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Previous work has shown that several products emerging from lipid peroxidation ( e.g. lipid hydroperoxides , lysophospholipids , oxidized cholesterol ) are able to reduce NO production in macrophages .
	manualset3
126676	5	405543	13	NULL	NULL	0	NULL	lysophospholipids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous work has shown that several products emerging from lipid peroxidation ( e.g. lipid hydroperoxides , lysophospholipids , oxidized cholesterol ) are able to reduce NO production in macrophages .
	manualset3
126677	6	405543	13	NULL	NULL	0	NULL	oxidized cholesterol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous work has shown that several products emerging from lipid peroxidation ( e.g. lipid hydroperoxides , lysophospholipids , oxidized cholesterol ) are able to reduce NO production in macrophages .
	manualset3
126678	7	405543	13	NULL	NULL	0	NULL	NO production 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous work has shown that several products emerging from lipid peroxidation ( e.g. lipid hydroperoxides , lysophospholipids , oxidized cholesterol ) are able to reduce NO production in macrophages .
	manualset3
126679	8	405543	13	NULL	NULL	0	NULL	macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous work has shown that several products emerging from lipid peroxidation ( e.g. lipid hydroperoxides , lysophospholipids , oxidized cholesterol ) are able to reduce NO production in macrophages .
	manualset3
126680	1	405544	13	NULL	NULL	0	NULL	150 kDa glycoprotein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously , a 150 kDa glycoprotein has been strongly implicated in slug cell adhesion and the present work suggests that additional glycoprotein ( s ) are involved .
	manualset3
126681	2	405544	13	NULL	NULL	0	NULL	slug cell adhesion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously , a 150 kDa glycoprotein has been strongly implicated in slug cell adhesion and the present work suggests that additional glycoprotein ( s ) are involved .
	manualset3
126682	3	405544	13	NULL	NULL	0	NULL	work	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously , a 150 kDa glycoprotein has been strongly implicated in slug cell adhesion and the present work suggests that additional glycoprotein ( s ) are involved .
	manualset3
126683	4	405544	13	NULL	NULL	0	NULL	glycoprotein ( s )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously , a 150 kDa glycoprotein has been strongly implicated in slug cell adhesion and the present work suggests that additional glycoprotein ( s ) are involved .
	manualset3
126684	1	405545	13	NULL	NULL	0	NULL	thymosin beta ( 10 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously , we and others have shown that thymosin beta ( 10 ) acts as an actin-mediated tumor suppressor .
	manualset3
126686	3	405545	13	NULL	NULL	0	NULL	actin-mediated tumor suppressor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously , we and others have shown that thymosin beta ( 10 ) acts as an actin-mediated tumor suppressor .
	manualset3
126687	1	405546	13	NULL	NULL	0	NULL	collaboration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously , we found that collaboration of reactive nitrogen intermediates ( RNI ) and free fatty acids ( FFA ) plays crucial roles in the expression of macrophage ( Mphi ) antimicrobial activity against Mycobacterium tuberculosis ( MTB ) .
	manualset3
126688	2	405546	13	NULL	NULL	0	NULL	reactive nitrogen intermediates ( RNI ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously , we found that collaboration of reactive nitrogen intermediates ( RNI ) and free fatty acids ( FFA ) plays crucial roles in the expression of macrophage ( Mphi ) antimicrobial activity against Mycobacterium tuberculosis ( MTB ) .
	manualset3
126689	3	405546	13	NULL	NULL	0	NULL	free fatty acids ( FFA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously , we found that collaboration of reactive nitrogen intermediates ( RNI ) and free fatty acids ( FFA ) plays crucial roles in the expression of macrophage ( Mphi ) antimicrobial activity against Mycobacterium tuberculosis ( MTB ) .
	manualset3
126690	4	405546	13	NULL	NULL	0	NULL	crucial roles	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously , we found that collaboration of reactive nitrogen intermediates ( RNI ) and free fatty acids ( FFA ) plays crucial roles in the expression of macrophage ( Mphi ) antimicrobial activity against Mycobacterium tuberculosis ( MTB ) .
	manualset3
126691	5	405546	13	NULL	NULL	0	NULL	expression of macrophage ( Mphi )	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously , we found that collaboration of reactive nitrogen intermediates ( RNI ) and free fatty acids ( FFA ) plays crucial roles in the expression of macrophage ( Mphi ) antimicrobial activity against Mycobacterium tuberculosis ( MTB ) .
	manualset3
126692	6	405546	13	NULL	NULL	0	NULL	antimicrobial activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously , we found that collaboration of reactive nitrogen intermediates ( RNI ) and free fatty acids ( FFA ) plays crucial roles in the expression of macrophage ( Mphi ) antimicrobial activity against Mycobacterium tuberculosis ( MTB ) .
	manualset3
126693	7	405546	13	NULL	NULL	0	NULL	Mycobacterium tuberculosis ( MTB ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously , we found that collaboration of reactive nitrogen intermediates ( RNI ) and free fatty acids ( FFA ) plays crucial roles in the expression of macrophage ( Mphi ) antimicrobial activity against Mycobacterium tuberculosis ( MTB ) .
	manualset3
126694	1	405547	13	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously , we reported that in rats , GABA ( A ) and glycine receptor immunoreactivity increased markedly in multiple brain stem respiratory nuclei around postnatal days ( P ) 12-13 , a critical period when abrupt neurochemical , metabolic , ventilatory , and electrophysiological changes occur in the respiratory network and when the system is under greater inhibition than excitation .
	manualset3
126695	2	405547	13	NULL	NULL	0	NULL	 GABA ( A ) receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously , we reported that in rats , GABA ( A ) and glycine receptor immunoreactivity increased markedly in multiple brain stem respiratory nuclei around postnatal days ( P ) 12-13 , a critical period when abrupt neurochemical , metabolic , ventilatory , and electrophysiological changes occur in the respiratory network and when the system is under greater inhibition than excitation .
	manualset3
126696	3	405547	13	NULL	NULL	0	NULL	glycine receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously , we reported that in rats , GABA ( A ) and glycine receptor immunoreactivity increased markedly in multiple brain stem respiratory nuclei around postnatal days ( P ) 12-13 , a critical period when abrupt neurochemical , metabolic , ventilatory , and electrophysiological changes occur in the respiratory network and when the system is under greater inhibition than excitation .
	manualset3
126697	4	405547	13	NULL	NULL	0	NULL	immunoreactivity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously , we reported that in rats , GABA ( A ) and glycine receptor immunoreactivity increased markedly in multiple brain stem respiratory nuclei around postnatal days ( P ) 12-13 , a critical period when abrupt neurochemical , metabolic , ventilatory , and electrophysiological changes occur in the respiratory network and when the system is under greater inhibition than excitation .
	manualset3
126698	5	405547	13	NULL	NULL	0	NULL	multiple brain stem respiratory nuclei	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously , we reported that in rats , GABA ( A ) and glycine receptor immunoreactivity increased markedly in multiple brain stem respiratory nuclei around postnatal days ( P ) 12-13 , a critical period when abrupt neurochemical , metabolic , ventilatory , and electrophysiological changes occur in the respiratory network and when the system is under greater inhibition than excitation .
	manualset3
126699	6	405547	13	NULL	NULL	0	NULL	postnatal days ( P ) 12-13	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously , we reported that in rats , GABA ( A ) and glycine receptor immunoreactivity increased markedly in multiple brain stem respiratory nuclei around postnatal days ( P ) 12-13 , a critical period when abrupt neurochemical , metabolic , ventilatory , and electrophysiological changes occur in the respiratory network and when the system is under greater inhibition than excitation .
	manualset3
126700	7	405547	13	NULL	NULL	0	NULL	period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously , we reported that in rats , GABA ( A ) and glycine receptor immunoreactivity increased markedly in multiple brain stem respiratory nuclei around postnatal days ( P ) 12-13 , a critical period when abrupt neurochemical , metabolic , ventilatory , and electrophysiological changes occur in the respiratory network and when the system is under greater inhibition than excitation .
	manualset3
126701	8	405547	13	NULL	NULL	0	NULL	neurochemical changes 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously , we reported that in rats , GABA ( A ) and glycine receptor immunoreactivity increased markedly in multiple brain stem respiratory nuclei around postnatal days ( P ) 12-13 , a critical period when abrupt neurochemical , metabolic , ventilatory , and electrophysiological changes occur in the respiratory network and when the system is under greater inhibition than excitation .
	manualset3
126702	9	405547	13	NULL	NULL	0	NULL	metabolic changes 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously , we reported that in rats , GABA ( A ) and glycine receptor immunoreactivity increased markedly in multiple brain stem respiratory nuclei around postnatal days ( P ) 12-13 , a critical period when abrupt neurochemical , metabolic , ventilatory , and electrophysiological changes occur in the respiratory network and when the system is under greater inhibition than excitation .
	manualset3
126703	10	405547	13	NULL	NULL	0	NULL	ventilatory changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously , we reported that in rats , GABA ( A ) and glycine receptor immunoreactivity increased markedly in multiple brain stem respiratory nuclei around postnatal days ( P ) 12-13 , a critical period when abrupt neurochemical , metabolic , ventilatory , and electrophysiological changes occur in the respiratory network and when the system is under greater inhibition than excitation .
	manualset3
126704	11	405547	13	NULL	NULL	0	NULL	electrophysiological changes 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously , we reported that in rats , GABA ( A ) and glycine receptor immunoreactivity increased markedly in multiple brain stem respiratory nuclei around postnatal days ( P ) 12-13 , a critical period when abrupt neurochemical , metabolic , ventilatory , and electrophysiological changes occur in the respiratory network and when the system is under greater inhibition than excitation .
	manualset3
126705	12	405547	13	NULL	NULL	0	NULL	respiratory network 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously , we reported that in rats , GABA ( A ) and glycine receptor immunoreactivity increased markedly in multiple brain stem respiratory nuclei around postnatal days ( P ) 12-13 , a critical period when abrupt neurochemical , metabolic , ventilatory , and electrophysiological changes occur in the respiratory network and when the system is under greater inhibition than excitation .
	manualset3
126706	13	405547	13	NULL	NULL	0	NULL	system 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously , we reported that in rats , GABA ( A ) and glycine receptor immunoreactivity increased markedly in multiple brain stem respiratory nuclei around postnatal days ( P ) 12-13 , a critical period when abrupt neurochemical , metabolic , ventilatory , and electrophysiological changes occur in the respiratory network and when the system is under greater inhibition than excitation .
	manualset3
126707	14	405547	13	NULL	NULL	0	NULL	inhibition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously , we reported that in rats , GABA ( A ) and glycine receptor immunoreactivity increased markedly in multiple brain stem respiratory nuclei around postnatal days ( P ) 12-13 , a critical period when abrupt neurochemical , metabolic , ventilatory , and electrophysiological changes occur in the respiratory network and when the system is under greater inhibition than excitation .
	manualset3
126708	15	405547	13	NULL	NULL	0	NULL	excitation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously , we reported that in rats , GABA ( A ) and glycine receptor immunoreactivity increased markedly in multiple brain stem respiratory nuclei around postnatal days ( P ) 12-13 , a critical period when abrupt neurochemical , metabolic , ventilatory , and electrophysiological changes occur in the respiratory network and when the system is under greater inhibition than excitation .
	manualset3
126709	1	405548	13	NULL	NULL	0	NULL	NMR data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously reported NMR data of three of these derivatives were corrected and the NMR data for the other three derivatives not studied previously were completely assigned on the basis of the basic 1D and 2D NMR experiments and molecular modeling .
	manualset3
126710	2	405548	13	NULL	NULL	NULL	NULL	three of these derivatives 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Previously reported NMR data of three of these derivatives were corrected and the NMR data for the other three derivatives not studied previously were completely assigned on the basis of the basic 1D and 2D NMR experiments and molecular modeling .
	manualset3
126711	3	405548	13	NULL	NULL	0	NULL	NMR data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously reported NMR data of three of these derivatives were corrected and the NMR data for the other three derivatives not studied previously were completely assigned on the basis of the basic 1D and 2D NMR experiments and molecular modeling .
	manualset3
126712	4	405548	13	NULL	NULL	NULL	NULL	three derivatives 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Previously reported NMR data of three of these derivatives were corrected and the NMR data for the other three derivatives not studied previously were completely assigned on the basis of the basic 1D and 2D NMR experiments and molecular modeling .
	manualset3
126713	5	405548	13	NULL	NULL	0	NULL	basis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously reported NMR data of three of these derivatives were corrected and the NMR data for the other three derivatives not studied previously were completely assigned on the basis of the basic 1D and 2D NMR experiments and molecular modeling .
	manualset3
126714	6	405548	13	NULL	NULL	0	NULL	basic 1D NMR experiments 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously reported NMR data of three of these derivatives were corrected and the NMR data for the other three derivatives not studied previously were completely assigned on the basis of the basic 1D and 2D NMR experiments and molecular modeling .
	manualset3
126715	7	405548	13	NULL	NULL	0	NULL	basic 2D NMR experiments 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously reported NMR data of three of these derivatives were corrected and the NMR data for the other three derivatives not studied previously were completely assigned on the basis of the basic 1D and 2D NMR experiments and molecular modeling .
	manualset3
126716	8	405548	13	NULL	NULL	0	NULL	molecular modeling 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Previously reported NMR data of three of these derivatives were corrected and the NMR data for the other three derivatives not studied previously were completely assigned on the basis of the basic 1D and 2D NMR experiments and molecular modeling .
	manualset3
126717	1	405549	13	NULL	NULL	0	NULL	Primary Hyperchylomicronemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary Hyperchylomicronemia is known as a syndrome in which the accumulation of chylomicron occurs in the circulation .
	manualset3
126718	2	405549	13	NULL	NULL	0	NULL	syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary Hyperchylomicronemia is known as a syndrome in which the accumulation of chylomicron occurs in the circulation .
	manualset3
126719	3	405549	13	NULL	NULL	0	NULL	accumulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary Hyperchylomicronemia is known as a syndrome in which the accumulation of chylomicron occurs in the circulation .
	manualset3
126720	4	405549	13	NULL	NULL	0	NULL	chylomicron	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary Hyperchylomicronemia is known as a syndrome in which the accumulation of chylomicron occurs in the circulation .
	manualset3
126721	5	405549	13	NULL	NULL	0	NULL	circulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary Hyperchylomicronemia is known as a syndrome in which the accumulation of chylomicron occurs in the circulation .
	manualset3
126722	1	405550	13	NULL	NULL	NULL	NULL	Primary carcinoma of the lung	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Primary carcinoma of the lung .
	manualset3
126724	1	405551	13	NULL	NULL	0	NULL	Primary cilia	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary cilia are required for cerebellar development and Shh-dependent expansion of progenitor pool .
	manualset3
126725	2	405551	13	NULL	NULL	0	NULL	cerebellar development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary cilia are required for cerebellar development and Shh-dependent expansion of progenitor pool .
	manualset3
126726	3	405551	13	NULL	NULL	0	NULL	 Shh-dependent expansion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary cilia are required for cerebellar development and Shh-dependent expansion of progenitor pool .
	manualset3
126727	4	405551	13	NULL	NULL	0	NULL	progenitor pool 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary cilia are required for cerebellar development and Shh-dependent expansion of progenitor pool .
	manualset3
126728	1	405552	13	NULL	NULL	0	NULL	Primary congenital glaucoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary congenital glaucoma : making strides in genetic testing , early detection and treatment .
	manualset3
126729	2	405552	13	NULL	NULL	0	NULL	strides	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary congenital glaucoma : making strides in genetic testing , early detection and treatment .
	manualset3
126730	3	405552	13	NULL	NULL	0	NULL	genetic testing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary congenital glaucoma : making strides in genetic testing , early detection and treatment .
	manualset3
126731	4	405552	13	NULL	NULL	0	NULL	detection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary congenital glaucoma : making strides in genetic testing , early detection and treatment .
	manualset3
126732	5	405552	13	NULL	NULL	0	NULL	treatment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary congenital glaucoma : making strides in genetic testing , early detection and treatment .
	manualset3
126733	1	405553	13	NULL	NULL	0	NULL	Primary cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary cultures of freshly iDCs were successfully maintained for 28 days in plastic dishes with RPMI 1640 culture medium .
	manualset3
126734	2	405553	13	NULL	NULL	0	NULL	iDCs 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary cultures of freshly iDCs were successfully maintained for 28 days in plastic dishes with RPMI 1640 culture medium .
	manualset3
126735	3	405553	13	NULL	NULL	0	NULL	 28 days	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary cultures of freshly iDCs were successfully maintained for 28 days in plastic dishes with RPMI 1640 culture medium .
	manualset3
126736	4	405553	13	NULL	NULL	0	NULL	plastic dishes	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary cultures of freshly iDCs were successfully maintained for 28 days in plastic dishes with RPMI 1640 culture medium .
	manualset3
126737	5	405553	13	NULL	NULL	0	NULL	RPMI 1640 culture medium 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary cultures of freshly iDCs were successfully maintained for 28 days in plastic dishes with RPMI 1640 culture medium .
	manualset3
126738	1	405554	13	NULL	NULL	0	NULL	Primary lymphedema 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary lymphedema may occur at any phase of life but it most commonly appears at puberty .
	manualset3
126739	2	405554	13	NULL	NULL	0	NULL	phase of life	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary lymphedema may occur at any phase of life but it most commonly appears at puberty .
	manualset3
126740	3	405554	13	NULL	NULL	0	NULL	puberty 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary lymphedema may occur at any phase of life but it most commonly appears at puberty .
	manualset3
126741	1	405555	13	NULL	NULL	0	NULL	Primary mucinous adenocarcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary mucinous adenocarcinoma of the bladder with signet-ring cells : case report .
	manualset3
126742	2	405555	13	NULL	NULL	0	NULL	bladder 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary mucinous adenocarcinoma of the bladder with signet-ring cells : case report .
	manualset3
126743	3	405555	13	NULL	NULL	0	NULL	signet-ring cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary mucinous adenocarcinoma of the bladder with signet-ring cells : case report .
	manualset3
126744	4	405555	13	NULL	NULL	0	NULL	case report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary mucinous adenocarcinoma of the bladder with signet-ring cells : case report .
	manualset3
126745	1	405556	13	NULL	NULL	0	NULL	Primary osseous tumors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary osseous tumors of the spine , in contrast , are rare conditions but may demonstrate typical imaging findings .
	manualset3
126746	2	405556	13	NULL	NULL	0	NULL	spine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary osseous tumors of the spine , in contrast , are rare conditions but may demonstrate typical imaging findings .
	manualset3
126747	3	405556	13	NULL	NULL	0	NULL	rare conditions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary osseous tumors of the spine , in contrast , are rare conditions but may demonstrate typical imaging findings .
	manualset3
126748	4	405556	13	NULL	NULL	0	NULL	typical imaging findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary osseous tumors of the spine , in contrast , are rare conditions but may demonstrate typical imaging findings .
	manualset3
126749	1	405557	13	NULL	NULL	0	NULL	Primary tumor excision	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary tumor excision in stage IV breast cancer at diagnosis without influence on survival : a retrospective analysis and review of the literature .
	manualset3
126750	2	405557	13	NULL	NULL	0	NULL	stage IV breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary tumor excision in stage IV breast cancer at diagnosis without influence on survival : a retrospective analysis and review of the literature .
	manualset3
126751	3	405557	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary tumor excision in stage IV breast cancer at diagnosis without influence on survival : a retrospective analysis and review of the literature .
	manualset3
126752	4	405557	13	NULL	NULL	0	NULL	 influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary tumor excision in stage IV breast cancer at diagnosis without influence on survival : a retrospective analysis and review of the literature .
	manualset3
126753	5	405557	13	NULL	NULL	0	NULL	 survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary tumor excision in stage IV breast cancer at diagnosis without influence on survival : a retrospective analysis and review of the literature .
	manualset3
126754	6	405557	13	NULL	NULL	0	NULL	retrospective analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary tumor excision in stage IV breast cancer at diagnosis without influence on survival : a retrospective analysis and review of the literature .
	manualset3
126755	7	405557	13	NULL	NULL	0	NULL	review	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary tumor excision in stage IV breast cancer at diagnosis without influence on survival : a retrospective analysis and review of the literature .
	manualset3
126756	8	405557	13	NULL	NULL	0	NULL	literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary tumor excision in stage IV breast cancer at diagnosis without influence on survival : a retrospective analysis and review of the literature .
	manualset3
126757	1	405558	13	NULL	NULL	NULL	NULL	Primary non-Hodgkin 's lymphoma of the brain	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Primary non-Hodgkin 's lymphoma of the brain is rare .
	manualset3
126759	1	405559	13	NULL	NULL	0	NULL	Primates 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Primates are also effective seed dispersers .
	manualset3
126760	2	405559	13	NULL	NULL	0	NULL	seed dispersers	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Primates are also effective seed dispersers .
	manualset3
126761	1	405560	13	NULL	NULL	0	NULL	Primers	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Primers designed from a consensus sequence have been used to obtain a fragment of 560 nucleotides , including the complete coding sequence of 456 nucleotides .
	manualset3
126762	2	405560	13	NULL	NULL	0	NULL	consensus sequence 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Primers designed from a consensus sequence have been used to obtain a fragment of 560 nucleotides , including the complete coding sequence of 456 nucleotides .
	manualset3
126763	3	405560	13	NULL	NULL	0	NULL	fragment of 560 nucleotides	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Primers designed from a consensus sequence have been used to obtain a fragment of 560 nucleotides , including the complete coding sequence of 456 nucleotides .
	manualset3
126764	4	405560	13	NULL	NULL	0	NULL	coding sequence 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Primers designed from a consensus sequence have been used to obtain a fragment of 560 nucleotides , including the complete coding sequence of 456 nucleotides .
	manualset3
126765	5	405560	13	NULL	NULL	0	NULL	456 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Primers designed from a consensus sequence have been used to obtain a fragment of 560 nucleotides , including the complete coding sequence of 456 nucleotides .
	manualset3
126766	6	405560	13	NULL	NULL	0	NULL	nucleotides	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Primers designed from a consensus sequence have been used to obtain a fragment of 560 nucleotides , including the complete coding sequence of 456 nucleotides .
	manualset3
126767	1	405561	13	NULL	NULL	0	NULL	Principles	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Principles and guidelines for surgeons -- management of symptomatic breast cancer .
	manualset3
126768	2	405561	13	NULL	NULL	0	NULL	guidelines	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Principles and guidelines for surgeons -- management of symptomatic breast cancer .
	manualset3
126769	3	405561	13	NULL	NULL	0	NULL	surgeons	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Principles and guidelines for surgeons -- management of symptomatic breast cancer .
	manualset3
126770	4	405561	13	NULL	NULL	0	NULL	 management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Principles and guidelines for surgeons -- management of symptomatic breast cancer .
	manualset3
126771	5	405561	13	NULL	NULL	0	NULL	symptomatic breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Principles and guidelines for surgeons -- management of symptomatic breast cancer .
	manualset3
126772	1	405562	13	NULL	NULL	0	NULL	Principles of prevention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Principles of prevention of cardiovascular disease .
	manualset3
126773	2	405562	13	NULL	NULL	0	NULL	cardiovascular disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Principles of prevention of cardiovascular disease .
	manualset3
126774	1	405563	13	NULL	NULL	NULL	NULL	Principles 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Principles of these stacking schemes are explained , new procedures and instrumental arrangements are discussed , and all contributions involving stacking principles that have been published since the year 2000 are surveyed .
	manualset3
126775	2	405563	13	NULL	NULL	0	NULL	stacking schemes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Principles of these stacking schemes are explained , new procedures and instrumental arrangements are discussed , and all contributions involving stacking principles that have been published since the year 2000 are surveyed .
	manualset3
126776	3	405563	13	NULL	NULL	0	NULL	new procedures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Principles of these stacking schemes are explained , new procedures and instrumental arrangements are discussed , and all contributions involving stacking principles that have been published since the year 2000 are surveyed .
	manualset3
126777	4	405563	13	NULL	NULL	0	NULL	instrumental arrangements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Principles of these stacking schemes are explained , new procedures and instrumental arrangements are discussed , and all contributions involving stacking principles that have been published since the year 2000 are surveyed .
	manualset3
126778	5	405563	13	NULL	NULL	0	NULL	contributions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Principles of these stacking schemes are explained , new procedures and instrumental arrangements are discussed , and all contributions involving stacking principles that have been published since the year 2000 are surveyed .
	manualset3
126779	6	405563	13	NULL	NULL	0	NULL	principles	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Principles of these stacking schemes are explained , new procedures and instrumental arrangements are discussed , and all contributions involving stacking principles that have been published since the year 2000 are surveyed .
	manualset3
126780	7	405563	13	NULL	NULL	0	NULL	year 2000	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Principles of these stacking schemes are explained , new procedures and instrumental arrangements are discussed , and all contributions involving stacking principles that have been published since the year 2000 are surveyed .
	manualset3
126781	1	405564	13	NULL	NULL	0	NULL	Prion diseases 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Prion diseases are characterized by deposits of abnormal conformers of the PrP protein .
	manualset3
126782	2	405564	13	NULL	NULL	0	NULL	deposits	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Prion diseases are characterized by deposits of abnormal conformers of the PrP protein .
	manualset3
126783	3	405564	13	NULL	NULL	0	NULL	abnormal conformers	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Prion diseases are characterized by deposits of abnormal conformers of the PrP protein .
	manualset3
126784	4	405564	13	NULL	NULL	0	NULL	PrP protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Prion diseases are characterized by deposits of abnormal conformers of the PrP protein .
	manualset3
126785	1	405565	13	NULL	NULL	0	NULL	linear relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A linear relationship was found between the retention volumes of these cells , except that of erythrocytes , on a PEG 20M-Sepharose column and their delta log K values determined in the presence or absence of sodium chloride both at the isoelectric points and at pH 7.5 .
	manualset3
126786	2	405565	13	NULL	NULL	0	NULL	retention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A linear relationship was found between the retention volumes of these cells , except that of erythrocytes , on a PEG 20M-Sepharose column and their delta log K values determined in the presence or absence of sodium chloride both at the isoelectric points and at pH 7.5 .
	manualset3
126787	3	405565	13	NULL	NULL	0	NULL	volumes	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A linear relationship was found between the retention volumes of these cells , except that of erythrocytes , on a PEG 20M-Sepharose column and their delta log K values determined in the presence or absence of sodium chloride both at the isoelectric points and at pH 7.5 .
	manualset3
126788	4	405565	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A linear relationship was found between the retention volumes of these cells , except that of erythrocytes , on a PEG 20M-Sepharose column and their delta log K values determined in the presence or absence of sodium chloride both at the isoelectric points and at pH 7.5 .
	manualset3
126789	5	405565	13	NULL	NULL	0	NULL	erythrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A linear relationship was found between the retention volumes of these cells , except that of erythrocytes , on a PEG 20M-Sepharose column and their delta log K values determined in the presence or absence of sodium chloride both at the isoelectric points and at pH 7.5 .
	manualset3
126790	6	405565	13	NULL	NULL	0	NULL	PEG 20M-Sepharose column	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A linear relationship was found between the retention volumes of these cells , except that of erythrocytes , on a PEG 20M-Sepharose column and their delta log K values determined in the presence or absence of sodium chloride both at the isoelectric points and at pH 7.5 .
	manualset3
126791	7	405565	13	NULL	NULL	0	NULL	delta log K values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A linear relationship was found between the retention volumes of these cells , except that of erythrocytes , on a PEG 20M-Sepharose column and their delta log K values determined in the presence or absence of sodium chloride both at the isoelectric points and at pH 7.5 .
	manualset3
126792	8	405565	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A linear relationship was found between the retention volumes of these cells , except that of erythrocytes , on a PEG 20M-Sepharose column and their delta log K values determined in the presence or absence of sodium chloride both at the isoelectric points and at pH 7.5 .
	manualset3
126793	9	405565	13	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A linear relationship was found between the retention volumes of these cells , except that of erythrocytes , on a PEG 20M-Sepharose column and their delta log K values determined in the presence or absence of sodium chloride both at the isoelectric points and at pH 7.5 .
	manualset3
126794	10	405565	13	NULL	NULL	0	NULL	sodium chloride 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A linear relationship was found between the retention volumes of these cells , except that of erythrocytes , on a PEG 20M-Sepharose column and their delta log K values determined in the presence or absence of sodium chloride both at the isoelectric points and at pH 7.5 .
	manualset3
126795	11	405565	13	NULL	NULL	0	NULL	isoelectric points 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A linear relationship was found between the retention volumes of these cells , except that of erythrocytes , on a PEG 20M-Sepharose column and their delta log K values determined in the presence or absence of sodium chloride both at the isoelectric points and at pH 7.5 .
	manualset3
126796	12	405565	13	NULL	NULL	0	NULL	 pH 7.5	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A linear relationship was found between the retention volumes of these cells , except that of erythrocytes , on a PEG 20M-Sepharose column and their delta log K values determined in the presence or absence of sodium chloride both at the isoelectric points and at pH 7.5 .
	manualset3
126797	1	405566	13	NULL	NULL	0	NULL	culture	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prior culture with NMDA induced less effective alterations in both intracellular free Ca ( 2 + ) levels and mitochondrial membrane potentials after the addition of NMDA in striatal neurons .
	manualset3
126798	2	405566	13	NULL	NULL	0	NULL	NMDA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Prior culture with NMDA induced less effective alterations in both intracellular free Ca ( 2 + ) levels and mitochondrial membrane potentials after the addition of NMDA in striatal neurons .
	manualset3
126799	3	405566	13	NULL	NULL	0	NULL	alterations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prior culture with NMDA induced less effective alterations in both intracellular free Ca ( 2 + ) levels and mitochondrial membrane potentials after the addition of NMDA in striatal neurons .
	manualset3
126800	4	405566	13	NULL	NULL	0	NULL	intracellular free Ca ( 2 + ) levels 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Prior culture with NMDA induced less effective alterations in both intracellular free Ca ( 2 + ) levels and mitochondrial membrane potentials after the addition of NMDA in striatal neurons .
	manualset3
126801	5	405566	13	NULL	NULL	0	NULL	mitochondrial membrane potentials 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Prior culture with NMDA induced less effective alterations in both intracellular free Ca ( 2 + ) levels and mitochondrial membrane potentials after the addition of NMDA in striatal neurons .
	manualset3
126802	6	405566	13	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prior culture with NMDA induced less effective alterations in both intracellular free Ca ( 2 + ) levels and mitochondrial membrane potentials after the addition of NMDA in striatal neurons .
	manualset3
126803	7	405566	13	NULL	NULL	0	NULL	NMDA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Prior culture with NMDA induced less effective alterations in both intracellular free Ca ( 2 + ) levels and mitochondrial membrane potentials after the addition of NMDA in striatal neurons .
	manualset3
126804	8	405566	13	NULL	NULL	0	NULL	striatal neurons 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Prior culture with NMDA induced less effective alterations in both intracellular free Ca ( 2 + ) levels and mitochondrial membrane potentials after the addition of NMDA in striatal neurons .
	manualset3
126805	1	405567	13	NULL	NULL	0	NULL	99mTc-d , l-HMPAO labeled leucocyte scan	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prior to the 99mTc-d , l-HMPAO labeled leucocyte scan , all patients underwent a 99mTc-MDP bone scan .
	manualset3
126806	2	405567	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Prior to the 99mTc-d , l-HMPAO labeled leucocyte scan , all patients underwent a 99mTc-MDP bone scan .
	manualset3
126807	3	405567	13	NULL	NULL	0	NULL	99mTc-MDP bone scan	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prior to the 99mTc-d , l-HMPAO labeled leucocyte scan , all patients underwent a 99mTc-MDP bone scan .
	manualset3
126808	1	405568	13	NULL	NULL	NULL	NULL	Probability 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Probability of lymph node metastasis in small gastric cancer tumor : is it an indication for limited surgery ?
	manualset3
126809	2	405568	13	NULL	NULL	0	NULL	lymph node metastasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Probability of lymph node metastasis in small gastric cancer tumor : is it an indication for limited surgery ?
	manualset3
126810	3	405568	13	NULL	NULL	0	NULL	small gastric cancer tumor 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Probability of lymph node metastasis in small gastric cancer tumor : is it an indication for limited surgery ?
	manualset3
126811	4	405568	13	NULL	NULL	0	NULL	indication 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Probability of lymph node metastasis in small gastric cancer tumor : is it an indication for limited surgery ?
	manualset3
126812	5	405568	13	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Probability of lymph node metastasis in small gastric cancer tumor : is it an indication for limited surgery ?
	manualset3
126813	1	405569	13	NULL	NULL	0	NULL	Probability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Probability of skin conductance response ( SCR ) was analyzed for a sample of 79 undergraduate women , ranging in age from 18 to 25 years .
	manualset3
126814	2	405569	13	NULL	NULL	0	NULL	skin conductance response ( SCR )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Probability of skin conductance response ( SCR ) was analyzed for a sample of 79 undergraduate women , ranging in age from 18 to 25 years .
	manualset3
126815	3	405569	13	NULL	NULL	0	NULL	sample	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Probability of skin conductance response ( SCR ) was analyzed for a sample of 79 undergraduate women , ranging in age from 18 to 25 years .
	manualset3
126816	4	405569	13	NULL	NULL	0	NULL	79 undergraduate women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Probability of skin conductance response ( SCR ) was analyzed for a sample of 79 undergraduate women , ranging in age from 18 to 25 years .
	manualset3
126817	5	405569	13	NULL	NULL	0	NULL	age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Probability of skin conductance response ( SCR ) was analyzed for a sample of 79 undergraduate women , ranging in age from 18 to 25 years .
	manualset3
126818	6	405569	13	NULL	NULL	0	NULL	18 to 25 years	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Probability of skin conductance response ( SCR ) was analyzed for a sample of 79 undergraduate women , ranging in age from 18 to 25 years .
	manualset3
126819	1	405570	13	NULL	NULL	0	NULL	literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A literature search was conducted to evaluate laparoscopic retroperitoneal lymph node dissection ( RPLND ) in comparison to other modalities of treatment .
	manualset3
126820	2	405570	13	NULL	NULL	0	NULL	search	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A literature search was conducted to evaluate laparoscopic retroperitoneal lymph node dissection ( RPLND ) in comparison to other modalities of treatment .
	manualset3
126821	3	405570	13	NULL	NULL	0	NULL	laparoscopic retroperitoneal lymph node dissection ( RPLND )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A literature search was conducted to evaluate laparoscopic retroperitoneal lymph node dissection ( RPLND ) in comparison to other modalities of treatment .
	manualset3
126822	4	405570	13	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A literature search was conducted to evaluate laparoscopic retroperitoneal lymph node dissection ( RPLND ) in comparison to other modalities of treatment .
	manualset3
126823	5	405570	13	NULL	NULL	0	NULL	modalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A literature search was conducted to evaluate laparoscopic retroperitoneal lymph node dissection ( RPLND ) in comparison to other modalities of treatment .
	manualset3
126824	6	405570	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A literature search was conducted to evaluate laparoscopic retroperitoneal lymph node dissection ( RPLND ) in comparison to other modalities of treatment .
	manualset3
126825	1	405571	13	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Probably the foremost hypothesis of depression is the 5-hydroxytryptamine ( 5-HT , serotonin ) deficiency hypothesis .
	manualset3
126826	2	405571	13	NULL	NULL	0	NULL	depression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Probably the foremost hypothesis of depression is the 5-hydroxytryptamine ( 5-HT , serotonin ) deficiency hypothesis .
	manualset3
126827	3	405571	13	NULL	NULL	NULL	NULL	5-hydroxytryptamine ( 5-HT , serotonin ) deficiency hypothesis 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Probably the foremost hypothesis of depression is the 5-hydroxytryptamine ( 5-HT , serotonin ) deficiency hypothesis .
	manualset3
126829	1	405572	13	NULL	NULL	0	NULL	Probe analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Probe analysis revealed an increased copper deposit , particularly during the chronic copper intoxication , and a very high concentration of iron gradually accumulated .
	manualset3
126830	2	405572	13	NULL	NULL	NULL	NULL	copper deposit 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Probe analysis revealed an increased copper deposit , particularly during the chronic copper intoxication , and a very high concentration of iron gradually accumulated .
	manualset3
126831	3	405572	13	NULL	NULL	0	NULL	chronic copper intoxication 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Probe analysis revealed an increased copper deposit , particularly during the chronic copper intoxication , and a very high concentration of iron gradually accumulated .
	manualset3
126832	4	405572	13	NULL	NULL	0	NULL	concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Probe analysis revealed an increased copper deposit , particularly during the chronic copper intoxication , and a very high concentration of iron gradually accumulated .
	manualset3
126833	5	405572	13	NULL	NULL	0	NULL	iron 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Probe analysis revealed an increased copper deposit , particularly during the chronic copper intoxication , and a very high concentration of iron gradually accumulated .
	manualset3
126834	1	405573	13	NULL	NULL	0	NULL	depth	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Probing depth was reduced from a mean of 8.3 to 4.5 mm .
	manualset3
126835	2	405573	13	NULL	NULL	0	NULL	mean of 8.3 to 4.5 mm 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Probing depth was reduced from a mean of 8.3 to 4.5 mm .
	manualset3
126836	1	405574	13	NULL	NULL	0	NULL	molecular structure 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Probing molecular structure and structural changes of voltage-gated channel by expressing mutant channels in yeast and reconstituting them into planar membranes .
	manualset3
126837	2	405574	13	NULL	NULL	0	NULL	structural changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Probing molecular structure and structural changes of voltage-gated channel by expressing mutant channels in yeast and reconstituting them into planar membranes .
	manualset3
126838	3	405574	13	NULL	NULL	0	NULL	voltage-gated channel	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Probing molecular structure and structural changes of voltage-gated channel by expressing mutant channels in yeast and reconstituting them into planar membranes .
	manualset3
126839	4	405574	13	NULL	NULL	0	NULL	mutant channels	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Probing molecular structure and structural changes of voltage-gated channel by expressing mutant channels in yeast and reconstituting them into planar membranes .
	manualset3
126840	5	405574	13	NULL	NULL	0	NULL	yeast 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Probing molecular structure and structural changes of voltage-gated channel by expressing mutant channels in yeast and reconstituting them into planar membranes .
	manualset3
126841	6	405574	13	NULL	NULL	0	NULL	planar membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Probing molecular structure and structural changes of voltage-gated channel by expressing mutant channels in yeast and reconstituting them into planar membranes .
	manualset3
126842	1	405575	13	NULL	NULL	0	NULL	Probiotics	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Probiotics for pediatric antibiotic-associated diarrhea : a meta-analysis of randomized placebo-controlled trials .
	manualset3
126843	2	405575	13	NULL	NULL	0	NULL	pediatric antibiotic-associated diarrhea	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Probiotics for pediatric antibiotic-associated diarrhea : a meta-analysis of randomized placebo-controlled trials .
	manualset3
126844	3	405575	13	NULL	NULL	0	NULL	meta-analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Probiotics for pediatric antibiotic-associated diarrhea : a meta-analysis of randomized placebo-controlled trials .
	manualset3
126845	4	405575	13	NULL	NULL	0	NULL	randomized placebo-controlled trials	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Probiotics for pediatric antibiotic-associated diarrhea : a meta-analysis of randomized placebo-controlled trials .
	manualset3
126846	1	405576	13	NULL	NULL	0	NULL	Problems	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Problems in cell wall assembly .
	manualset3
126847	2	405576	13	NULL	NULL	0	NULL	cell wall assembly 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Problems in cell wall assembly .
	manualset3
126848	1	405577	13	NULL	NULL	0	NULL	rumen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A localized rumen buffering effect could not be excluded and could be linked with a higher amount of HCO3 recycled into the rumen .
	manualset3
126849	2	405577	13	NULL	NULL	0	NULL	buffering effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A localized rumen buffering effect could not be excluded and could be linked with a higher amount of HCO3 recycled into the rumen .
	manualset3
126850	3	405577	13	NULL	NULL	0	NULL	amount	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A localized rumen buffering effect could not be excluded and could be linked with a higher amount of HCO3 recycled into the rumen .
	manualset3
126851	4	405577	13	NULL	NULL	0	NULL	HCO3	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A localized rumen buffering effect could not be excluded and could be linked with a higher amount of HCO3 recycled into the rumen .
	manualset3
126852	5	405577	13	NULL	NULL	0	NULL	rumen 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A localized rumen buffering effect could not be excluded and could be linked with a higher amount of HCO3 recycled into the rumen .
	manualset3
126853	1	405578	13	NULL	NULL	0	NULL	Problems 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Problems related to innovations in the health care system and the susceptibility of medico-prophylactic institutions to advanced methodologies are discussed .
	manualset3
126854	2	405578	13	NULL	NULL	0	NULL	innovations	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Problems related to innovations in the health care system and the susceptibility of medico-prophylactic institutions to advanced methodologies are discussed .
	manualset3
126855	3	405578	13	NULL	NULL	0	NULL	 health care system	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Problems related to innovations in the health care system and the susceptibility of medico-prophylactic institutions to advanced methodologies are discussed .
	manualset3
126856	4	405578	13	NULL	NULL	0	NULL	susceptibility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Problems related to innovations in the health care system and the susceptibility of medico-prophylactic institutions to advanced methodologies are discussed .
	manualset3
126857	5	405578	13	NULL	NULL	0	NULL	medico-prophylactic institutions 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Problems related to innovations in the health care system and the susceptibility of medico-prophylactic institutions to advanced methodologies are discussed .
	manualset3
126858	6	405578	13	NULL	NULL	0	NULL	methodologies	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Problems related to innovations in the health care system and the susceptibility of medico-prophylactic institutions to advanced methodologies are discussed .
	manualset3
126859	1	405579	13	NULL	NULL	0	NULL	Procedure guideline 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Procedure guideline for radionuclide cystography in children .
	manualset3
126860	2	405579	13	NULL	NULL	0	NULL	radionuclide cystography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Procedure guideline for radionuclide cystography in children .
	manualset3
126861	3	405579	13	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Procedure guideline for radionuclide cystography in children .
	manualset3
126862	1	405580	13	NULL	NULL	0	NULL	Procedures 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Procedures involved in foot trimming , docking , castrating , dosing , dehorning , descenting , dewattling , and giving injections are discussed .
	manualset3
126863	2	405580	13	NULL	NULL	0	NULL	foot trimming	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Procedures involved in foot trimming , docking , castrating , dosing , dehorning , descenting , dewattling , and giving injections are discussed .
	manualset3
126864	3	405580	13	NULL	NULL	0	NULL	docking	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Procedures involved in foot trimming , docking , castrating , dosing , dehorning , descenting , dewattling , and giving injections are discussed .
	manualset3
126865	4	405580	13	NULL	NULL	0	NULL	castrating	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Procedures involved in foot trimming , docking , castrating , dosing , dehorning , descenting , dewattling , and giving injections are discussed .
	manualset3
126866	5	405580	13	NULL	NULL	0	NULL	dosing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Procedures involved in foot trimming , docking , castrating , dosing , dehorning , descenting , dewattling , and giving injections are discussed .
	manualset3
126867	6	405580	13	NULL	NULL	0	NULL	dehorning 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Procedures involved in foot trimming , docking , castrating , dosing , dehorning , descenting , dewattling , and giving injections are discussed .
	manualset3
126868	7	405580	13	NULL	NULL	0	NULL	descenting 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Procedures involved in foot trimming , docking , castrating , dosing , dehorning , descenting , dewattling , and giving injections are discussed .
	manualset3
126869	8	405580	13	NULL	NULL	0	NULL	dewattling 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Procedures involved in foot trimming , docking , castrating , dosing , dehorning , descenting , dewattling , and giving injections are discussed .
	manualset3
126870	9	405580	13	NULL	NULL	0	NULL	injections	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Procedures involved in foot trimming , docking , castrating , dosing , dehorning , descenting , dewattling , and giving injections are discussed .
	manualset3
126871	1	405581	13	NULL	NULL	0	NULL	Proceedings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceedings : Concentrations of plasma LH and FSH in cycling ewes following a single injection of 17beta-oestradiol .
	manualset3
126872	2	405581	13	NULL	NULL	0	NULL	Concentrations of plasma LH	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceedings : Concentrations of plasma LH and FSH in cycling ewes following a single injection of 17beta-oestradiol .
	manualset3
126873	3	405581	13	NULL	NULL	NULL	NULL	Concentrations of plasma FSH	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Proceedings : Concentrations of plasma LH and FSH in cycling ewes following a single injection of 17beta-oestradiol .
	manualset3
126874	4	405581	13	NULL	NULL	NULL	NULL	ewes	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Proceedings : Concentrations of plasma LH and FSH in cycling ewes following a single injection of 17beta-oestradiol .
	manualset3
126875	5	405581	13	NULL	NULL	NULL	NULL	injection	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Proceedings : Concentrations of plasma LH and FSH in cycling ewes following a single injection of 17beta-oestradiol .
	manualset3
126876	6	405581	13	NULL	NULL	0	NULL	17beta-oestradiol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceedings : Concentrations of plasma LH and FSH in cycling ewes following a single injection of 17beta-oestradiol .
	manualset3
126877	1	405582	13	NULL	NULL	0	NULL	Proceedings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceedings : Control of amylase secretion in the parotid gland .
	manualset3
126878	2	405582	13	NULL	NULL	0	NULL	Control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceedings : Control of amylase secretion in the parotid gland .
	manualset3
126879	3	405582	13	NULL	NULL	0	NULL	amylase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceedings : Control of amylase secretion in the parotid gland .
	manualset3
126880	4	405582	13	NULL	NULL	0	NULL	secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceedings : Control of amylase secretion in the parotid gland .
	manualset3
126881	5	405582	13	NULL	NULL	0	NULL	parotid gland	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceedings : Control of amylase secretion in the parotid gland .
	manualset3
126882	1	405583	13	NULL	NULL	0	NULL	Proceedings 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceedings : US experience with occupational safety and health legislation -- an industrial view .
	manualset3
126883	2	405583	13	NULL	NULL	0	NULL	US	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceedings : US experience with occupational safety and health legislation -- an industrial view .
	manualset3
126884	3	405583	13	NULL	NULL	0	NULL	experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceedings : US experience with occupational safety and health legislation -- an industrial view .
	manualset3
126885	4	405583	13	NULL	NULL	0	NULL	occupational safety	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceedings : US experience with occupational safety and health legislation -- an industrial view .
	manualset3
126886	5	405583	13	NULL	NULL	0	NULL	health legislation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceedings : US experience with occupational safety and health legislation -- an industrial view .
	manualset3
126887	6	405583	13	NULL	NULL	0	NULL	industrial view	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceedings : US experience with occupational safety and health legislation -- an industrial view .
	manualset3
126888	1	405584	13	NULL	NULL	0	NULL	Process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Process mapping the prevalence of salmonella contamination on pork carcass from slaughter to chilling : a systematic review approach .
	manualset3
126889	2	405584	13	NULL	NULL	0	NULL	prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Process mapping the prevalence of salmonella contamination on pork carcass from slaughter to chilling : a systematic review approach .
	manualset3
126890	3	405584	13	NULL	NULL	0	NULL	salmonella contamination	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Process mapping the prevalence of salmonella contamination on pork carcass from slaughter to chilling : a systematic review approach .
	manualset3
126891	4	405584	13	NULL	NULL	0	NULL	pork carcass	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Process mapping the prevalence of salmonella contamination on pork carcass from slaughter to chilling : a systematic review approach .
	manualset3
126892	5	405584	13	NULL	NULL	0	NULL	slaughter	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Process mapping the prevalence of salmonella contamination on pork carcass from slaughter to chilling : a systematic review approach .
	manualset3
126893	6	405584	13	NULL	NULL	0	NULL	systematic review approach	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Process mapping the prevalence of salmonella contamination on pork carcass from slaughter to chilling : a systematic review approach .
	manualset3
126894	1	405585	13	NULL	NULL	0	NULL	Procoagulant responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Procoagulant and prothrombotic responses of human endothelium to indomethacin and endotoxin in vitro .
	manualset3
126895	2	405585	13	NULL	NULL	0	NULL	prothrombotic responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Procoagulant and prothrombotic responses of human endothelium to indomethacin and endotoxin in vitro .
	manualset3
126896	3	405585	13	NULL	NULL	0	NULL	human endothelium	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Procoagulant and prothrombotic responses of human endothelium to indomethacin and endotoxin in vitro .
	manualset3
126897	4	405585	13	NULL	NULL	0	NULL	indomethacin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Procoagulant and prothrombotic responses of human endothelium to indomethacin and endotoxin in vitro .
	manualset3
126898	5	405585	13	NULL	NULL	0	NULL	endotoxin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Procoagulant and prothrombotic responses of human endothelium to indomethacin and endotoxin in vitro .
	manualset3
126899	1	405586	13	NULL	NULL	0	NULL	change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Producing change in attitudes toward abortion .
	manualset3
126900	2	405586	13	NULL	NULL	0	NULL	attitudes	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Producing change in attitudes toward abortion .
	manualset3
126901	3	405586	13	NULL	NULL	0	NULL	abortion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Producing change in attitudes toward abortion .
	manualset3
126902	1	405587	13	NULL	NULL	0	NULL	Production 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Production and characterization of partially purified extracellular thermostable - amylase by Bacillus subtilis in submerged fermentation ( SmF ) .
	manualset3
126903	2	405587	13	NULL	NULL	0	NULL	characterization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Production and characterization of partially purified extracellular thermostable - amylase by Bacillus subtilis in submerged fermentation ( SmF ) .
	manualset3
126904	3	405587	13	NULL	NULL	0	NULL	extracellular thermostable - amylase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Production and characterization of partially purified extracellular thermostable - amylase by Bacillus subtilis in submerged fermentation ( SmF ) .
	manualset3
126905	4	405587	13	NULL	NULL	0	NULL	Bacillus subtilis 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Production and characterization of partially purified extracellular thermostable - amylase by Bacillus subtilis in submerged fermentation ( SmF ) .
	manualset3
126906	5	405587	13	NULL	NULL	NULL	NULL	submerged fermentation ( SmF ) 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Production and characterization of partially purified extracellular thermostable - amylase by Bacillus subtilis in submerged fermentation ( SmF ) .
	manualset3
126907	1	405588	13	NULL	NULL	0	NULL	Production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Production and extraction optimization of xylanase from Aspergillus niger DFR-5 through solid-state-fermentation .
	manualset3
126908	2	405588	13	NULL	NULL	0	NULL	extraction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Production and extraction optimization of xylanase from Aspergillus niger DFR-5 through solid-state-fermentation .
	manualset3
126909	3	405588	13	NULL	NULL	0	NULL	optimization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Production and extraction optimization of xylanase from Aspergillus niger DFR-5 through solid-state-fermentation .
	manualset3
126910	4	405588	13	NULL	NULL	0	NULL	xylanase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Production and extraction optimization of xylanase from Aspergillus niger DFR-5 through solid-state-fermentation .
	manualset3
126911	5	405588	13	NULL	NULL	0	NULL	Aspergillus niger 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Production and extraction optimization of xylanase from Aspergillus niger DFR-5 through solid-state-fermentation .
	manualset3
126912	6	405588	13	NULL	NULL	0	NULL	DFR-5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Production and extraction optimization of xylanase from Aspergillus niger DFR-5 through solid-state-fermentation .
	manualset3
126913	7	405588	13	NULL	NULL	0	NULL	solid-state-fermentation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Production and extraction optimization of xylanase from Aspergillus niger DFR-5 through solid-state-fermentation .
	manualset3
126914	1	405589	13	NULL	NULL	0	NULL	logistic regression model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A logistic regression model adjusting for age , year of diagnosis , ethnicity , and duration of enrollment prior to diagnosis found that statistically significant predictors of more advanced stage of disease at diagnosis included young age , diagnosis after 1991 for non-Hispanic white women , and diagnosis prior to 1992 for Hispanic women .
	manualset3
126915	2	405589	13	NULL	NULL	0	NULL	age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A logistic regression model adjusting for age , year of diagnosis , ethnicity , and duration of enrollment prior to diagnosis found that statistically significant predictors of more advanced stage of disease at diagnosis included young age , diagnosis after 1991 for non-Hispanic white women , and diagnosis prior to 1992 for Hispanic women .
	manualset3
126916	3	405589	13	NULL	NULL	0	NULL	year 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	A logistic regression model adjusting for age , year of diagnosis , ethnicity , and duration of enrollment prior to diagnosis found that statistically significant predictors of more advanced stage of disease at diagnosis included young age , diagnosis after 1991 for non-Hispanic white women , and diagnosis prior to 1992 for Hispanic women .
	manualset3
126917	4	405589	13	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A logistic regression model adjusting for age , year of diagnosis , ethnicity , and duration of enrollment prior to diagnosis found that statistically significant predictors of more advanced stage of disease at diagnosis included young age , diagnosis after 1991 for non-Hispanic white women , and diagnosis prior to 1992 for Hispanic women .
	manualset3
126918	5	405589	13	NULL	NULL	0	NULL	ethnicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A logistic regression model adjusting for age , year of diagnosis , ethnicity , and duration of enrollment prior to diagnosis found that statistically significant predictors of more advanced stage of disease at diagnosis included young age , diagnosis after 1991 for non-Hispanic white women , and diagnosis prior to 1992 for Hispanic women .
	manualset3
126919	6	405589	13	NULL	NULL	0	NULL	duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A logistic regression model adjusting for age , year of diagnosis , ethnicity , and duration of enrollment prior to diagnosis found that statistically significant predictors of more advanced stage of disease at diagnosis included young age , diagnosis after 1991 for non-Hispanic white women , and diagnosis prior to 1992 for Hispanic women .
	manualset3
126920	7	405589	13	NULL	NULL	0	NULL	enrollment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A logistic regression model adjusting for age , year of diagnosis , ethnicity , and duration of enrollment prior to diagnosis found that statistically significant predictors of more advanced stage of disease at diagnosis included young age , diagnosis after 1991 for non-Hispanic white women , and diagnosis prior to 1992 for Hispanic women .
	manualset3
126921	8	405589	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A logistic regression model adjusting for age , year of diagnosis , ethnicity , and duration of enrollment prior to diagnosis found that statistically significant predictors of more advanced stage of disease at diagnosis included young age , diagnosis after 1991 for non-Hispanic white women , and diagnosis prior to 1992 for Hispanic women .
	manualset3
126922	9	405589	13	NULL	NULL	0	NULL	predictors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A logistic regression model adjusting for age , year of diagnosis , ethnicity , and duration of enrollment prior to diagnosis found that statistically significant predictors of more advanced stage of disease at diagnosis included young age , diagnosis after 1991 for non-Hispanic white women , and diagnosis prior to 1992 for Hispanic women .
	manualset3
126923	10	405589	13	NULL	NULL	0	NULL	stage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A logistic regression model adjusting for age , year of diagnosis , ethnicity , and duration of enrollment prior to diagnosis found that statistically significant predictors of more advanced stage of disease at diagnosis included young age , diagnosis after 1991 for non-Hispanic white women , and diagnosis prior to 1992 for Hispanic women .
	manualset3
126924	11	405589	13	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A logistic regression model adjusting for age , year of diagnosis , ethnicity , and duration of enrollment prior to diagnosis found that statistically significant predictors of more advanced stage of disease at diagnosis included young age , diagnosis after 1991 for non-Hispanic white women , and diagnosis prior to 1992 for Hispanic women .
	manualset3
126925	12	405589	13	NULL	NULL	NULL	NULL	young age	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A logistic regression model adjusting for age , year of diagnosis , ethnicity , and duration of enrollment prior to diagnosis found that statistically significant predictors of more advanced stage of disease at diagnosis included young age , diagnosis after 1991 for non-Hispanic white women , and diagnosis prior to 1992 for Hispanic women .
	manualset3
126926	13	405589	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A logistic regression model adjusting for age , year of diagnosis , ethnicity , and duration of enrollment prior to diagnosis found that statistically significant predictors of more advanced stage of disease at diagnosis included young age , diagnosis after 1991 for non-Hispanic white women , and diagnosis prior to 1992 for Hispanic women .
	manualset3
126927	14	405589	13	NULL	NULL	0	NULL	1991	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	A logistic regression model adjusting for age , year of diagnosis , ethnicity , and duration of enrollment prior to diagnosis found that statistically significant predictors of more advanced stage of disease at diagnosis included young age , diagnosis after 1991 for non-Hispanic white women , and diagnosis prior to 1992 for Hispanic women .
	manualset3
126928	15	405589	13	NULL	NULL	0	NULL	non-Hispanic white women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A logistic regression model adjusting for age , year of diagnosis , ethnicity , and duration of enrollment prior to diagnosis found that statistically significant predictors of more advanced stage of disease at diagnosis included young age , diagnosis after 1991 for non-Hispanic white women , and diagnosis prior to 1992 for Hispanic women .
	manualset3
126929	16	405589	13	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A logistic regression model adjusting for age , year of diagnosis , ethnicity , and duration of enrollment prior to diagnosis found that statistically significant predictors of more advanced stage of disease at diagnosis included young age , diagnosis after 1991 for non-Hispanic white women , and diagnosis prior to 1992 for Hispanic women .
	manualset3
126930	17	405589	13	NULL	NULL	0	NULL	1992 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	A logistic regression model adjusting for age , year of diagnosis , ethnicity , and duration of enrollment prior to diagnosis found that statistically significant predictors of more advanced stage of disease at diagnosis included young age , diagnosis after 1991 for non-Hispanic white women , and diagnosis prior to 1992 for Hispanic women .
	manualset3
126931	18	405589	13	NULL	NULL	0	NULL	Hispanic women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A logistic regression model adjusting for age , year of diagnosis , ethnicity , and duration of enrollment prior to diagnosis found that statistically significant predictors of more advanced stage of disease at diagnosis included young age , diagnosis after 1991 for non-Hispanic white women , and diagnosis prior to 1992 for Hispanic women .
	manualset3
126932	1	405590	13	NULL	NULL	0	NULL	Production 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of an inhibitor of rat mesangial cell growth by the glomerulus and its alteration in puromycin nephrosis .
	manualset3
126933	2	405590	13	NULL	NULL	0	NULL	inhibitor	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of an inhibitor of rat mesangial cell growth by the glomerulus and its alteration in puromycin nephrosis .
	manualset3
126934	3	405590	13	NULL	NULL	0	NULL	rat mesangial cell growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of an inhibitor of rat mesangial cell growth by the glomerulus and its alteration in puromycin nephrosis .
	manualset3
126935	4	405590	13	NULL	NULL	0	NULL	glomerulus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of an inhibitor of rat mesangial cell growth by the glomerulus and its alteration in puromycin nephrosis .
	manualset3
126936	5	405590	13	NULL	NULL	0	NULL	alteration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of an inhibitor of rat mesangial cell growth by the glomerulus and its alteration in puromycin nephrosis .
	manualset3
126937	6	405590	13	NULL	NULL	0	NULL	puromycin nephrosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of an inhibitor of rat mesangial cell growth by the glomerulus and its alteration in puromycin nephrosis .
	manualset3
126938	1	405591	13	NULL	NULL	0	NULL	Production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of antisera against oxytocin and lysine-vasopressin has prompted us to test their specificity against lysine-vasopressin , arginine-vasopressin , arginine-vasotocin , and oxytocin .
	manualset3
126939	2	405591	13	NULL	NULL	0	NULL	antisera against oxytocin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of antisera against oxytocin and lysine-vasopressin has prompted us to test their specificity against lysine-vasopressin , arginine-vasopressin , arginine-vasotocin , and oxytocin .
	manualset3
126940	3	405591	13	NULL	NULL	0	NULL	antisera against lysine-vasopressin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of antisera against oxytocin and lysine-vasopressin has prompted us to test their specificity against lysine-vasopressin , arginine-vasopressin , arginine-vasotocin , and oxytocin .
	manualset3
126941	4	405591	13	NULL	NULL	0	NULL	specificity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of antisera against oxytocin and lysine-vasopressin has prompted us to test their specificity against lysine-vasopressin , arginine-vasopressin , arginine-vasotocin , and oxytocin .
	manualset3
126942	5	405591	13	NULL	NULL	0	NULL	lysine-vasopressin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of antisera against oxytocin and lysine-vasopressin has prompted us to test their specificity against lysine-vasopressin , arginine-vasopressin , arginine-vasotocin , and oxytocin .
	manualset3
126943	6	405591	13	NULL	NULL	0	NULL	arginine-vasopressin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of antisera against oxytocin and lysine-vasopressin has prompted us to test their specificity against lysine-vasopressin , arginine-vasopressin , arginine-vasotocin , and oxytocin .
	manualset3
126944	7	405591	13	NULL	NULL	0	NULL	arginine-vasotocin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of antisera against oxytocin and lysine-vasopressin has prompted us to test their specificity against lysine-vasopressin , arginine-vasopressin , arginine-vasotocin , and oxytocin .
	manualset3
126945	8	405591	13	NULL	NULL	0	NULL	oxytocin 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of antisera against oxytocin and lysine-vasopressin has prompted us to test their specificity against lysine-vasopressin , arginine-vasopressin , arginine-vasotocin , and oxytocin .
	manualset3
126946	1	405592	13	NULL	NULL	0	NULL	Production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of hepatitis delta virus and suppression of helper hepatitis B virus in a human hepatoma cell line .
	manualset3
126947	2	405592	13	NULL	NULL	0	NULL	hepatitis delta virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of hepatitis delta virus and suppression of helper hepatitis B virus in a human hepatoma cell line .
	manualset3
126948	3	405592	13	NULL	NULL	0	NULL	suppression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of hepatitis delta virus and suppression of helper hepatitis B virus in a human hepatoma cell line .
	manualset3
126949	4	405592	13	NULL	NULL	0	NULL	helper hepatitis B virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of hepatitis delta virus and suppression of helper hepatitis B virus in a human hepatoma cell line .
	manualset3
126950	5	405592	13	NULL	NULL	0	NULL	human hepatoma cell line 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of hepatitis delta virus and suppression of helper hepatitis B virus in a human hepatoma cell line .
	manualset3
126951	1	405593	13	NULL	NULL	0	NULL	Production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of human tissue factor using the Pichia pastoris expression system .
	manualset3
126952	2	405593	13	NULL	NULL	0	NULL	human tissue factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of human tissue factor using the Pichia pastoris expression system .
	manualset3
126953	3	405593	13	NULL	NULL	0	NULL	Pichia pastoris 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of human tissue factor using the Pichia pastoris expression system .
	manualset3
126954	4	405593	13	NULL	NULL	0	NULL	expression system	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of human tissue factor using the Pichia pastoris expression system .
	manualset3
126955	1	405594	13	NULL	NULL	0	NULL	Production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of invertebrate predators closely tracked the increased production of their prey .
	manualset3
126956	2	405594	13	NULL	NULL	0	NULL	invertebrate predators 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of invertebrate predators closely tracked the increased production of their prey .
	manualset3
126957	3	405594	13	NULL	NULL	0	NULL	production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of invertebrate predators closely tracked the increased production of their prey .
	manualset3
126958	4	405594	13	NULL	NULL	0	NULL	prey 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of invertebrate predators closely tracked the increased production of their prey .
	manualset3
126959	1	405595	13	NULL	NULL	NULL	NULL	Production	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Production of nephritogenic autoantibodies , glomerular immune complex deposition , and cytokine overproduction have been postulated to contribute to the pathogenesis of LN .
	manualset3
126960	2	405595	13	NULL	NULL	0	NULL	nephritogenic autoantibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of nephritogenic autoantibodies , glomerular immune complex deposition , and cytokine overproduction have been postulated to contribute to the pathogenesis of LN .
	manualset3
126961	3	405595	13	NULL	NULL	0	NULL	glomerular immune complex deposition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of nephritogenic autoantibodies , glomerular immune complex deposition , and cytokine overproduction have been postulated to contribute to the pathogenesis of LN .
	manualset3
126962	4	405595	13	NULL	NULL	0	NULL	cytokine overproduction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of nephritogenic autoantibodies , glomerular immune complex deposition , and cytokine overproduction have been postulated to contribute to the pathogenesis of LN .
	manualset3
126963	5	405595	13	NULL	NULL	0	NULL	pathogenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of nephritogenic autoantibodies , glomerular immune complex deposition , and cytokine overproduction have been postulated to contribute to the pathogenesis of LN .
	manualset3
126964	6	405595	13	NULL	NULL	0	NULL	LN 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of nephritogenic autoantibodies , glomerular immune complex deposition , and cytokine overproduction have been postulated to contribute to the pathogenesis of LN .
	manualset3
126965	1	405596	13	NULL	NULL	0	NULL	Production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of resveratrol from p-coumaric acid in recombinant Saccharomyces cerevisiae expressing 4-coumarate : coenzyme A ligase and stilbene synthase genes .
	manualset3
126966	2	405596	13	NULL	NULL	0	NULL	resveratrol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of resveratrol from p-coumaric acid in recombinant Saccharomyces cerevisiae expressing 4-coumarate : coenzyme A ligase and stilbene synthase genes .
	manualset3
126967	3	405596	13	NULL	NULL	0	NULL	p-coumaric acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of resveratrol from p-coumaric acid in recombinant Saccharomyces cerevisiae expressing 4-coumarate : coenzyme A ligase and stilbene synthase genes .
	manualset3
126968	4	405596	13	NULL	NULL	0	NULL	recombinant Saccharomyces cerevisiae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of resveratrol from p-coumaric acid in recombinant Saccharomyces cerevisiae expressing 4-coumarate : coenzyme A ligase and stilbene synthase genes .
	manualset3
126969	5	405596	13	NULL	NULL	0	NULL	4-coumarate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of resveratrol from p-coumaric acid in recombinant Saccharomyces cerevisiae expressing 4-coumarate : coenzyme A ligase and stilbene synthase genes .
	manualset3
126970	6	405596	13	NULL	NULL	0	NULL	coenzyme A ligase genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of resveratrol from p-coumaric acid in recombinant Saccharomyces cerevisiae expressing 4-coumarate : coenzyme A ligase and stilbene synthase genes .
	manualset3
126971	7	405596	13	NULL	NULL	0	NULL	stilbene synthase gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of resveratrol from p-coumaric acid in recombinant Saccharomyces cerevisiae expressing 4-coumarate : coenzyme A ligase and stilbene synthase genes .
	manualset3
126972	1	405597	13	NULL	NULL	0	NULL	Production 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of the indamine dye by the peroxidase reaction is rapid but it may be stopped by lowering the pH to 3.0 .
	manualset3
126973	2	405597	13	NULL	NULL	0	NULL	indamine dye	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of the indamine dye by the peroxidase reaction is rapid but it may be stopped by lowering the pH to 3.0 .
	manualset3
126974	3	405597	13	NULL	NULL	0	NULL	peroxidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of the indamine dye by the peroxidase reaction is rapid but it may be stopped by lowering the pH to 3.0 .
	manualset3
126975	4	405597	13	NULL	NULL	0	NULL	reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of the indamine dye by the peroxidase reaction is rapid but it may be stopped by lowering the pH to 3.0 .
	manualset3
126976	5	405597	13	NULL	NULL	0	NULL	pH	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of the indamine dye by the peroxidase reaction is rapid but it may be stopped by lowering the pH to 3.0 .
	manualset3
126977	6	405597	13	NULL	NULL	0	NULL	3.0	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of the indamine dye by the peroxidase reaction is rapid but it may be stopped by lowering the pH to 3.0 .
	manualset3
126978	1	405598	13	NULL	NULL	0	NULL	Production 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Production performance was monitored throughout the pig 's lifetime .
	manualset3
126979	2	405598	13	NULL	NULL	0	NULL	performance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Production performance was monitored throughout the pig 's lifetime .
	manualset3
126980	3	405598	13	NULL	NULL	0	NULL	pig 's lifetime	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Production performance was monitored throughout the pig 's lifetime .
	manualset3
126981	1	405599	13	NULL	NULL	0	NULL	Productive ER import	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Productive ER import could be reinstated by increasing the amount of alpha-helical domains , whereas more effective ER signal sequences had only a minor effect on ER import efficiency of unstructured polypeptides .
	manualset3
126982	2	405599	13	NULL	NULL	0	NULL	amount	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Productive ER import could be reinstated by increasing the amount of alpha-helical domains , whereas more effective ER signal sequences had only a minor effect on ER import efficiency of unstructured polypeptides .
	manualset3
126983	3	405599	13	NULL	NULL	0	NULL	alpha-helical domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Productive ER import could be reinstated by increasing the amount of alpha-helical domains , whereas more effective ER signal sequences had only a minor effect on ER import efficiency of unstructured polypeptides .
	manualset3
126984	4	405599	13	NULL	NULL	NULL	NULL	ER signal sequences	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Productive ER import could be reinstated by increasing the amount of alpha-helical domains , whereas more effective ER signal sequences had only a minor effect on ER import efficiency of unstructured polypeptides .
	manualset3
126985	5	405599	13	NULL	NULL	0	NULL	effect 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Productive ER import could be reinstated by increasing the amount of alpha-helical domains , whereas more effective ER signal sequences had only a minor effect on ER import efficiency of unstructured polypeptides .
	manualset3
126986	6	405599	13	NULL	NULL	0	NULL	ER import efficiency	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Productive ER import could be reinstated by increasing the amount of alpha-helical domains , whereas more effective ER signal sequences had only a minor effect on ER import efficiency of unstructured polypeptides .
	manualset3
126987	7	405599	13	NULL	NULL	0	NULL	polypeptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Productive ER import could be reinstated by increasing the amount of alpha-helical domains , whereas more effective ER signal sequences had only a minor effect on ER import efficiency of unstructured polypeptides .
	manualset3
126988	1	405600	13	NULL	NULL	0	NULL	longitudinal study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A longitudinal study of maternal folate and vitamin B12 status in pregnancy and postpartum , with the same infant markers at 6 months of age .
	manualset3
126989	2	405600	13	NULL	NULL	0	NULL	maternal folate status 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A longitudinal study of maternal folate and vitamin B12 status in pregnancy and postpartum , with the same infant markers at 6 months of age .
	manualset3
126990	3	405600	13	NULL	NULL	0	NULL	maternal vitamin B12 status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A longitudinal study of maternal folate and vitamin B12 status in pregnancy and postpartum , with the same infant markers at 6 months of age .
	manualset3
126991	4	405600	13	NULL	NULL	0	NULL	pregnancy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A longitudinal study of maternal folate and vitamin B12 status in pregnancy and postpartum , with the same infant markers at 6 months of age .
	manualset3
126992	5	405600	13	NULL	NULL	0	NULL	postpartum	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A longitudinal study of maternal folate and vitamin B12 status in pregnancy and postpartum , with the same infant markers at 6 months of age .
	manualset3
126993	6	405600	13	NULL	NULL	0	NULL	infant markers 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A longitudinal study of maternal folate and vitamin B12 status in pregnancy and postpartum , with the same infant markers at 6 months of age .
	manualset3
126994	7	405600	13	NULL	NULL	0	NULL	6 months of age 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A longitudinal study of maternal folate and vitamin B12 status in pregnancy and postpartum , with the same infant markers at 6 months of age .
	manualset3
126995	1	405601	13	NULL	NULL	0	NULL	Productivity costs 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Productivity costs are a far more important economic factor , especially due to reduced employment , which are enhanced by the early age of diagnose onset .
	manualset3
126996	2	405601	13	NULL	NULL	0	NULL	economic factor	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Productivity costs are a far more important economic factor , especially due to reduced employment , which are enhanced by the early age of diagnose onset .
	manualset3
126997	3	405601	13	NULL	NULL	0	NULL	employment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Productivity costs are a far more important economic factor , especially due to reduced employment , which are enhanced by the early age of diagnose onset .
	manualset3
126998	4	405601	13	NULL	NULL	0	NULL	early age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Productivity costs are a far more important economic factor , especially due to reduced employment , which are enhanced by the early age of diagnose onset .
	manualset3
126999	5	405601	13	NULL	NULL	0	NULL	onset	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Productivity costs are a far more important economic factor , especially due to reduced employment , which are enhanced by the early age of diagnose onset .
	manualset3
127000	1	405602	13	NULL	NULL	0	NULL	Professional norms	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Professional norms and physician attitudes toward euthanasia .
	manualset3
127001	2	405602	13	NULL	NULL	0	NULL	 physician attitudes	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Professional norms and physician attitudes toward euthanasia .
	manualset3
127002	3	405602	13	NULL	NULL	NULL	NULL	euthanasia	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Professional norms and physician attitudes toward euthanasia .
	manualset3
127003	1	405603	13	NULL	NULL	0	NULL	counterfeit medicines 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Profiling of counterfeit medicines by vibrational spectroscopy .
	manualset3
127004	2	405603	13	NULL	NULL	0	NULL	vibrational spectroscopy 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Profiling of counterfeit medicines by vibrational spectroscopy .
	manualset3
127006	1	405604	13	NULL	NULL	0	NULL	Progesterone 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Progesterone increases protein synthesis in medium-sized ( 0.8 mm in diameter ) oocytes without inducing meiosis .
	manualset3
127008	3	405604	13	NULL	NULL	0	NULL	protein synthesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Progesterone increases protein synthesis in medium-sized ( 0.8 mm in diameter ) oocytes without inducing meiosis .
	manualset3
127009	4	405604	13	NULL	NULL	0	NULL	0.8 mm in diameter 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Progesterone increases protein synthesis in medium-sized ( 0.8 mm in diameter ) oocytes without inducing meiosis .
	manualset3
127010	5	405604	13	NULL	NULL	0	NULL	medium-sized oocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Progesterone increases protein synthesis in medium-sized ( 0.8 mm in diameter ) oocytes without inducing meiosis .
	manualset3
127011	6	405604	13	NULL	NULL	0	NULL	meiosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Progesterone increases protein synthesis in medium-sized ( 0.8 mm in diameter ) oocytes without inducing meiosis .
	manualset3
127012	1	405605	13	NULL	NULL	0	NULL	Prognosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognosis of HER2 over-expressing gastric cancer patients with liver metastasis .
	manualset3
127013	2	405605	13	NULL	NULL	0	NULL	HER2 over-expressing gastric cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognosis of HER2 over-expressing gastric cancer patients with liver metastasis .
	manualset3
127014	3	405605	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognosis of HER2 over-expressing gastric cancer patients with liver metastasis .
	manualset3
127015	4	405605	13	NULL	NULL	0	NULL	liver metastasis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognosis of HER2 over-expressing gastric cancer patients with liver metastasis .
	manualset3
127016	1	405606	13	NULL	NULL	0	NULL	Prognosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognosis of vesticoureteral reflux : a dissenting view .
	manualset3
127017	2	405606	13	NULL	NULL	0	NULL	vesticoureteral reflux 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognosis of vesticoureteral reflux : a dissenting view .
	manualset3
127018	3	405606	13	NULL	NULL	0	NULL	view 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognosis of vesticoureteral reflux : a dissenting view .
	manualset3
127019	1	405607	13	NULL	NULL	0	NULL	Prognosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognosis with chest pain and normal thallium-201 exercise scintigrams .
	manualset3
127020	2	405607	13	NULL	NULL	0	NULL	chest pain 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognosis with chest pain and normal thallium-201 exercise scintigrams .
	manualset3
127021	3	405607	13	NULL	NULL	0	NULL	thallium-201 exercise scintigrams	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognosis with chest pain and normal thallium-201 exercise scintigrams .
	manualset3
127022	1	405608	13	NULL	NULL	0	NULL	Prognostic factors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic factors in atrioventricular block complicating acute myocardial infarction .
	manualset3
127023	2	405608	13	NULL	NULL	0	NULL	atrioventricular block 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic factors in atrioventricular block complicating acute myocardial infarction .
	manualset3
127024	3	405608	13	NULL	NULL	0	NULL	acute myocardial infarction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic factors in atrioventricular block complicating acute myocardial infarction .
	manualset3
127025	1	405609	13	NULL	NULL	0	NULL	Prognostic factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic factors of resected node-positive lung cancer : location , extent of nodal metastases , and multimodal treatment .
	manualset3
127026	2	405609	13	NULL	NULL	0	NULL	resected node-positive lung cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic factors of resected node-positive lung cancer : location , extent of nodal metastases , and multimodal treatment .
	manualset3
127027	3	405609	13	NULL	NULL	0	NULL	location	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic factors of resected node-positive lung cancer : location , extent of nodal metastases , and multimodal treatment .
	manualset3
127028	4	405609	13	NULL	NULL	0	NULL	extent of nodal metastases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic factors of resected node-positive lung cancer : location , extent of nodal metastases , and multimodal treatment .
	manualset3
127029	5	405609	13	NULL	NULL	0	NULL	multimodal treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic factors of resected node-positive lung cancer : location , extent of nodal metastases , and multimodal treatment .
	manualset3
127031	2	405610	13	NULL	NULL	NULL	NULL	loss of heterozygosity ( LOH ) analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A loss of heterozygosity ( LOH ) analysis of 32 medulloblastomas with paired normal DNA samples was performed with 4 microsatellite markers flanking the GSK-3beta locus ; LOH with at least one marker was identified in 7 tumors .
	manualset3
127032	3	405610	13	NULL	NULL	0	NULL	32 medulloblastomas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A loss of heterozygosity ( LOH ) analysis of 32 medulloblastomas with paired normal DNA samples was performed with 4 microsatellite markers flanking the GSK-3beta locus ; LOH with at least one marker was identified in 7 tumors .
	manualset3
127033	4	405610	13	NULL	NULL	0	NULL	DNA samples	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A loss of heterozygosity ( LOH ) analysis of 32 medulloblastomas with paired normal DNA samples was performed with 4 microsatellite markers flanking the GSK-3beta locus ; LOH with at least one marker was identified in 7 tumors .
	manualset3
127034	5	405610	13	NULL	NULL	0	NULL	4 microsatellite markers flanking	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A loss of heterozygosity ( LOH ) analysis of 32 medulloblastomas with paired normal DNA samples was performed with 4 microsatellite markers flanking the GSK-3beta locus ; LOH with at least one marker was identified in 7 tumors .
	manualset3
127035	6	405610	13	NULL	NULL	0	NULL	GSK-3beta locus	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A loss of heterozygosity ( LOH ) analysis of 32 medulloblastomas with paired normal DNA samples was performed with 4 microsatellite markers flanking the GSK-3beta locus ; LOH with at least one marker was identified in 7 tumors .
	manualset3
127036	7	405610	13	NULL	NULL	0	NULL	LOH 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A loss of heterozygosity ( LOH ) analysis of 32 medulloblastomas with paired normal DNA samples was performed with 4 microsatellite markers flanking the GSK-3beta locus ; LOH with at least one marker was identified in 7 tumors .
	manualset3
127037	8	405610	13	NULL	NULL	0	NULL	marker	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A loss of heterozygosity ( LOH ) analysis of 32 medulloblastomas with paired normal DNA samples was performed with 4 microsatellite markers flanking the GSK-3beta locus ; LOH with at least one marker was identified in 7 tumors .
	manualset3
127038	9	405610	13	NULL	NULL	0	NULL	7 tumors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A loss of heterozygosity ( LOH ) analysis of 32 medulloblastomas with paired normal DNA samples was performed with 4 microsatellite markers flanking the GSK-3beta locus ; LOH with at least one marker was identified in 7 tumors .
	manualset3
127039	1	405611	13	NULL	NULL	0	NULL	Prognostic significance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic significance of molecular upstaging of paraffin-embedded sentinel lymph nodes in melanoma patients .
	manualset3
127040	2	405611	13	NULL	NULL	0	NULL	molecular upstaging 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic significance of molecular upstaging of paraffin-embedded sentinel lymph nodes in melanoma patients .
	manualset3
127041	3	405611	13	NULL	NULL	0	NULL	paraffin-embedded sentinel lymph nodes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic significance of molecular upstaging of paraffin-embedded sentinel lymph nodes in melanoma patients .
	manualset3
127042	4	405611	13	NULL	NULL	0	NULL	melanoma patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic significance of molecular upstaging of paraffin-embedded sentinel lymph nodes in melanoma patients .
	manualset3
127043	1	405612	13	NULL	NULL	0	NULL	Prognostic value	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic value of epidermal growth factor expression in breast cancer .
	manualset3
127044	2	405612	13	NULL	NULL	0	NULL	epidermal growth factor expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic value of epidermal growth factor expression in breast cancer .
	manualset3
127045	3	405612	13	NULL	NULL	0	NULL	breast cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic value of epidermal growth factor expression in breast cancer .
	manualset3
127046	1	405613	13	NULL	NULL	0	NULL	Prognostic value	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic value of platelet derived growth factor alpha receptor expression in grade 2 astrocytomas and oligoastrocytomas .
	manualset3
127047	2	405613	13	NULL	NULL	0	NULL	platelet derived growth factor alpha receptor expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic value of platelet derived growth factor alpha receptor expression in grade 2 astrocytomas and oligoastrocytomas .
	manualset3
127048	3	405613	13	NULL	NULL	0	NULL	grade 2 astrocytomas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic value of platelet derived growth factor alpha receptor expression in grade 2 astrocytomas and oligoastrocytomas .
	manualset3
127049	4	405613	13	NULL	NULL	0	NULL	oligoastrocytomas 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic value of platelet derived growth factor alpha receptor expression in grade 2 astrocytomas and oligoastrocytomas .
	manualset3
127050	1	405614	13	NULL	NULL	0	NULL	chromosome end formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Programmed chromosome end formation resulting from DNA fragmentation and telomeric repeat addition as well as programmed internal sequence elimination occur extensively during differentiation of macronuclear genomes from micronuclear chromosomal sets in ciliated protozoa .
	manualset3
127051	2	405614	13	NULL	NULL	0	NULL	DNA fragmentation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Programmed chromosome end formation resulting from DNA fragmentation and telomeric repeat addition as well as programmed internal sequence elimination occur extensively during differentiation of macronuclear genomes from micronuclear chromosomal sets in ciliated protozoa .
	manualset3
127052	3	405614	13	NULL	NULL	0	NULL	telomeric repeat addition 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Programmed chromosome end formation resulting from DNA fragmentation and telomeric repeat addition as well as programmed internal sequence elimination occur extensively during differentiation of macronuclear genomes from micronuclear chromosomal sets in ciliated protozoa .
	manualset3
127053	4	405614	13	NULL	NULL	0	NULL	internal sequence elimination	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Programmed chromosome end formation resulting from DNA fragmentation and telomeric repeat addition as well as programmed internal sequence elimination occur extensively during differentiation of macronuclear genomes from micronuclear chromosomal sets in ciliated protozoa .
	manualset3
127054	5	405614	13	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Programmed chromosome end formation resulting from DNA fragmentation and telomeric repeat addition as well as programmed internal sequence elimination occur extensively during differentiation of macronuclear genomes from micronuclear chromosomal sets in ciliated protozoa .
	manualset3
127055	6	405614	13	NULL	NULL	0	NULL	macronuclear genomes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Programmed chromosome end formation resulting from DNA fragmentation and telomeric repeat addition as well as programmed internal sequence elimination occur extensively during differentiation of macronuclear genomes from micronuclear chromosomal sets in ciliated protozoa .
	manualset3
127056	7	405614	13	NULL	NULL	0	NULL	micronuclear chromosomal sets	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Programmed chromosome end formation resulting from DNA fragmentation and telomeric repeat addition as well as programmed internal sequence elimination occur extensively during differentiation of macronuclear genomes from micronuclear chromosomal sets in ciliated protozoa .
	manualset3
127057	8	405614	13	NULL	NULL	0	NULL	ciliated protozoa	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Programmed chromosome end formation resulting from DNA fragmentation and telomeric repeat addition as well as programmed internal sequence elimination occur extensively during differentiation of macronuclear genomes from micronuclear chromosomal sets in ciliated protozoa .
	manualset3
127058	1	405615	13	NULL	NULL	0	NULL	Progress 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Progress in the foundations of mathematics has made it possible to formulate all thinkable mathematical concepts , algorithms and proofs in one language and in an impeccable way .
	manualset3
127059	2	405615	13	NULL	NULL	0	NULL	foundations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Progress in the foundations of mathematics has made it possible to formulate all thinkable mathematical concepts , algorithms and proofs in one language and in an impeccable way .
	manualset3
127060	3	405615	13	NULL	NULL	0	NULL	mathematics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Progress in the foundations of mathematics has made it possible to formulate all thinkable mathematical concepts , algorithms and proofs in one language and in an impeccable way .
	manualset3
127061	4	405615	13	NULL	NULL	0	NULL	mathematical concepts	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Progress in the foundations of mathematics has made it possible to formulate all thinkable mathematical concepts , algorithms and proofs in one language and in an impeccable way .
	manualset3
127062	5	405615	13	NULL	NULL	0	NULL	algorithms	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Progress in the foundations of mathematics has made it possible to formulate all thinkable mathematical concepts , algorithms and proofs in one language and in an impeccable way .
	manualset3
127063	6	405615	13	NULL	NULL	0	NULL	proofs 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Progress in the foundations of mathematics has made it possible to formulate all thinkable mathematical concepts , algorithms and proofs in one language and in an impeccable way .
	manualset3
127064	7	405615	13	NULL	NULL	0	NULL	language	Language												NULL		0	NULL	NULL	NULL	NULL	NULL	Progress in the foundations of mathematics has made it possible to formulate all thinkable mathematical concepts , algorithms and proofs in one language and in an impeccable way .
	manualset3
127065	8	405615	13	NULL	NULL	0	NULL	impeccable way	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Progress in the foundations of mathematics has made it possible to formulate all thinkable mathematical concepts , algorithms and proofs in one language and in an impeccable way .
	manualset3
127066	1	405616	13	NULL	NULL	0	NULL	Progress	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Progress in detection and identification is largely a result of improvements in separation and isolation , especially by gas chromatography , together with the introduction of mass spectrometry .
	manualset3
127067	2	405616	13	NULL	NULL	0	NULL	detection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Progress in detection and identification is largely a result of improvements in separation and isolation , especially by gas chromatography , together with the introduction of mass spectrometry .
	manualset3
127068	3	405616	13	NULL	NULL	0	NULL	identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Progress in detection and identification is largely a result of improvements in separation and isolation , especially by gas chromatography , together with the introduction of mass spectrometry .
	manualset3
127069	4	405616	13	NULL	NULL	0	NULL	result 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Progress in detection and identification is largely a result of improvements in separation and isolation , especially by gas chromatography , together with the introduction of mass spectrometry .
	manualset3
127070	5	405616	13	NULL	NULL	0	NULL	improvements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Progress in detection and identification is largely a result of improvements in separation and isolation , especially by gas chromatography , together with the introduction of mass spectrometry .
	manualset3
127071	6	405616	13	NULL	NULL	0	NULL	separation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Progress in detection and identification is largely a result of improvements in separation and isolation , especially by gas chromatography , together with the introduction of mass spectrometry .
	manualset3
127072	7	405616	13	NULL	NULL	0	NULL	isolation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Progress in detection and identification is largely a result of improvements in separation and isolation , especially by gas chromatography , together with the introduction of mass spectrometry .
	manualset3
127073	8	405616	13	NULL	NULL	0	NULL	gas chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Progress in detection and identification is largely a result of improvements in separation and isolation , especially by gas chromatography , together with the introduction of mass spectrometry .
	manualset3
127074	9	405616	13	NULL	NULL	0	NULL	introduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Progress in detection and identification is largely a result of improvements in separation and isolation , especially by gas chromatography , together with the introduction of mass spectrometry .
	manualset3
127075	10	405616	13	NULL	NULL	0	NULL	mass spectrometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Progress in detection and identification is largely a result of improvements in separation and isolation , especially by gas chromatography , together with the introduction of mass spectrometry .
	manualset3
127076	1	405617	13	NULL	NULL	0	NULL	level of FVIII	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A low level of FVIII : C seems to be a forecast of failure .
	manualset3
127077	2	405617	13	NULL	NULL	0	NULL	C	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A low level of FVIII : C seems to be a forecast of failure .
	manualset3
127078	3	405617	13	NULL	NULL	0	NULL	failure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A low level of FVIII : C seems to be a forecast of failure .
	manualset3
128812	4	405617	13	NULL	NULL	0	NULL	forecast	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A low level of FVIII : C seems to be a forecast of failure .
	manualset3
127079	1	405618	13	NULL	NULL	0	NULL	Progressive systemic myeloma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Progressive systemic myeloma led to her death 11 years after presentation and 9 years after seed implantation .
	manualset3
127080	2	405618	13	NULL	NULL	0	NULL	death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Progressive systemic myeloma led to her death 11 years after presentation and 9 years after seed implantation .
	manualset3
127081	3	405618	13	NULL	NULL	0	NULL	11 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Progressive systemic myeloma led to her death 11 years after presentation and 9 years after seed implantation .
	manualset3
127082	4	405618	13	NULL	NULL	0	NULL	presentation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Progressive systemic myeloma led to her death 11 years after presentation and 9 years after seed implantation .
	manualset3
127083	5	405618	13	NULL	NULL	0	NULL	9 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Progressive systemic myeloma led to her death 11 years after presentation and 9 years after seed implantation .
	manualset3
127085	7	405618	13	NULL	NULL	NULL	NULL	seed implantation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Progressive systemic myeloma led to her death 11 years after presentation and 9 years after seed implantation .
	manualset3
127086	1	405619	13	NULL	NULL	0	NULL	Projection printing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Projection printing of 3-dimensional tissue scaffolds .
	manualset3
127087	2	405619	13	NULL	NULL	NULL	NULL	3-dimensional tissue scaffolds	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Projection printing of 3-dimensional tissue scaffolds .
	manualset3
127088	1	405620	13	NULL	NULL	0	NULL	Prokaryotic RNase P 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Prokaryotic RNase P will function with a minihelix consisting of the acceptor stem connected directly to the T stem-loop .
	manualset3
127089	2	405620	13	NULL	NULL	0	NULL	minihelix 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Prokaryotic RNase P will function with a minihelix consisting of the acceptor stem connected directly to the T stem-loop .
	manualset3
127090	3	405620	13	NULL	NULL	0	NULL	acceptor stem	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Prokaryotic RNase P will function with a minihelix consisting of the acceptor stem connected directly to the T stem-loop .
	manualset3
127091	4	405620	13	NULL	NULL	0	NULL	T stem-loop	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Prokaryotic RNase P will function with a minihelix consisting of the acceptor stem connected directly to the T stem-loop .
	manualset3
127092	1	405621	13	NULL	NULL	0	NULL	Prolactin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolactin release by the cultured metastatic tumor cells was more potently inhibited by CV 205-502 than by bromocriptine .
	manualset3
127093	2	405621	13	NULL	NULL	0	NULL	release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolactin release by the cultured metastatic tumor cells was more potently inhibited by CV 205-502 than by bromocriptine .
	manualset3
127094	3	405621	13	NULL	NULL	0	NULL	metastatic tumor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolactin release by the cultured metastatic tumor cells was more potently inhibited by CV 205-502 than by bromocriptine .
	manualset3
127095	4	405621	13	NULL	NULL	0	NULL	CV 205-502	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolactin release by the cultured metastatic tumor cells was more potently inhibited by CV 205-502 than by bromocriptine .
	manualset3
127096	5	405621	13	NULL	NULL	0	NULL	bromocriptine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolactin release by the cultured metastatic tumor cells was more potently inhibited by CV 205-502 than by bromocriptine .
	manualset3
127097	1	405622	13	NULL	NULL	0	NULL	Prolactin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolactin treatment alone had no effect ; however , it potentiated the increase in CYP1B1 mRNA and protein expression by LH .
	manualset3
127098	2	405622	13	NULL	NULL	0	NULL	treatment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolactin treatment alone had no effect ; however , it potentiated the increase in CYP1B1 mRNA and protein expression by LH .
	manualset3
127099	3	405622	13	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolactin treatment alone had no effect ; however , it potentiated the increase in CYP1B1 mRNA and protein expression by LH .
	manualset3
127100	4	405622	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolactin treatment alone had no effect ; however , it potentiated the increase in CYP1B1 mRNA and protein expression by LH .
	manualset3
127101	5	405622	13	NULL	NULL	0	NULL	CYP1B1 mRNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolactin treatment alone had no effect ; however , it potentiated the increase in CYP1B1 mRNA and protein expression by LH .
	manualset3
127102	6	405622	13	NULL	NULL	0	NULL	CYP1B1 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolactin treatment alone had no effect ; however , it potentiated the increase in CYP1B1 mRNA and protein expression by LH .
	manualset3
127103	7	405622	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolactin treatment alone had no effect ; however , it potentiated the increase in CYP1B1 mRNA and protein expression by LH .
	manualset3
127104	8	405622	13	NULL	NULL	0	NULL	LH	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolactin treatment alone had no effect ; however , it potentiated the increase in CYP1B1 mRNA and protein expression by LH .
	manualset3
127105	1	405623	13	NULL	NULL	0	NULL	Prolapse 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolapse is possibly unrelated etiologically to cough , or chronic laryngeal or respiratory tract infection .
	manualset3
127106	2	405623	13	NULL	NULL	0	NULL	chronic laryngeal infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolapse is possibly unrelated etiologically to cough , or chronic laryngeal or respiratory tract infection .
	manualset3
127107	3	405623	13	NULL	NULL	0	NULL	respiratory tract infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolapse is possibly unrelated etiologically to cough , or chronic laryngeal or respiratory tract infection .
	manualset3
128813	4	405623	13	NULL	NULL	0	NULL	cough	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolapse is possibly unrelated etiologically to cough , or chronic laryngeal or respiratory tract infection .
	manualset3
127108	1	405624	13	NULL	NULL	0	NULL	melting point	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A low melting point cadmium free fusible lead alloy suitable for custom radiotherapy shielding blocks is described .
	manualset3
127109	2	405624	13	NULL	NULL	0	NULL	cadmium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	A low melting point cadmium free fusible lead alloy suitable for custom radiotherapy shielding blocks is described .
	manualset3
127110	3	405624	13	NULL	NULL	0	NULL	lead alloy	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	A low melting point cadmium free fusible lead alloy suitable for custom radiotherapy shielding blocks is described .
	manualset3
127111	4	405624	13	NULL	NULL	0	NULL	custom radiotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A low melting point cadmium free fusible lead alloy suitable for custom radiotherapy shielding blocks is described .
	manualset3
127112	5	405624	13	NULL	NULL	0	NULL	shielding blocks 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A low melting point cadmium free fusible lead alloy suitable for custom radiotherapy shielding blocks is described .
	manualset3
127113	1	405625	13	NULL	NULL	0	NULL	Proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Proliferation of NRICC was evaluated following stable knock down of 17-HSD3 .
	manualset3
127114	2	405625	13	NULL	NULL	0	NULL	NRICC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Proliferation of NRICC was evaluated following stable knock down of 17-HSD3 .
	manualset3
127115	3	405625	13	NULL	NULL	0	NULL	17-HSD3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Proliferation of NRICC was evaluated following stable knock down of 17-HSD3 .
	manualset3
128814	4	405625	13	NULL	NULL	0	NULL	knock down	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Proliferation of NRICC was evaluated following stable knock down of 17-HSD3 .
	manualset3
127116	1	405626	13	NULL	NULL	0	NULL	Proliferative activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Proliferative activity of gastric epithelial cells in Helicobacter pylori infected children .
	manualset3
127117	2	405626	13	NULL	NULL	0	NULL	gastric epithelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Proliferative activity of gastric epithelial cells in Helicobacter pylori infected children .
	manualset3
127118	3	405626	13	NULL	NULL	0	NULL	Helicobacter pylori 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Proliferative activity of gastric epithelial cells in Helicobacter pylori infected children .
	manualset3
127119	4	405626	13	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Proliferative activity of gastric epithelial cells in Helicobacter pylori infected children .
	manualset3
127120	1	405627	13	NULL	NULL	0	NULL	Prolongation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolongation of corneal allograft survival by topical application of everolimus in experimental keratoplasty .
	manualset3
127121	2	405627	13	NULL	NULL	0	NULL	corneal allograft survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolongation of corneal allograft survival by topical application of everolimus in experimental keratoplasty .
	manualset3
127122	3	405627	13	NULL	NULL	0	NULL	topical application	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolongation of corneal allograft survival by topical application of everolimus in experimental keratoplasty .
	manualset3
127123	4	405627	13	NULL	NULL	0	NULL	everolimus 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolongation of corneal allograft survival by topical application of everolimus in experimental keratoplasty .
	manualset3
127124	5	405627	13	NULL	NULL	0	NULL	experimental keratoplasty	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolongation of corneal allograft survival by topical application of everolimus in experimental keratoplasty .
	manualset3
127125	1	405628	13	NULL	NULL	0	NULL	antibiotic therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged antibiotic therapy is required in cases with extensive damage of lung tissue .
	manualset3
127126	2	405628	13	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged antibiotic therapy is required in cases with extensive damage of lung tissue .
	manualset3
127127	3	405628	13	NULL	NULL	0	NULL	extensive damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged antibiotic therapy is required in cases with extensive damage of lung tissue .
	manualset3
127128	4	405628	13	NULL	NULL	0	NULL	lung tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged antibiotic therapy is required in cases with extensive damage of lung tissue .
	manualset3
127129	1	405629	13	NULL	NULL	0	NULL	Prolonged exercise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged exercise ( 60 min ) performed on a bicycle ergometer in aerobic conditions led to strong activation of the fibrinolytic system ( euglobulin lysis time ( ELT ) fell from 208 to 88 min ) and a slight increase in platelet count ( PC ) but did not cause significant changes in platelet factor 4 ( PF 4 ) and platelet aggregate ratio , recalcification ( RT ) , and prothrombin time ( PT ) .
	manualset3
127130	2	405629	13	NULL	NULL	0	NULL	60 min	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged exercise ( 60 min ) performed on a bicycle ergometer in aerobic conditions led to strong activation of the fibrinolytic system ( euglobulin lysis time ( ELT ) fell from 208 to 88 min ) and a slight increase in platelet count ( PC ) but did not cause significant changes in platelet factor 4 ( PF 4 ) and platelet aggregate ratio , recalcification ( RT ) , and prothrombin time ( PT ) .
	manualset3
127131	3	405629	13	NULL	NULL	0	NULL	bicycle ergometer	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged exercise ( 60 min ) performed on a bicycle ergometer in aerobic conditions led to strong activation of the fibrinolytic system ( euglobulin lysis time ( ELT ) fell from 208 to 88 min ) and a slight increase in platelet count ( PC ) but did not cause significant changes in platelet factor 4 ( PF 4 ) and platelet aggregate ratio , recalcification ( RT ) , and prothrombin time ( PT ) .
	manualset3
127132	4	405629	13	NULL	NULL	0	NULL	aerobic conditions 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged exercise ( 60 min ) performed on a bicycle ergometer in aerobic conditions led to strong activation of the fibrinolytic system ( euglobulin lysis time ( ELT ) fell from 208 to 88 min ) and a slight increase in platelet count ( PC ) but did not cause significant changes in platelet factor 4 ( PF 4 ) and platelet aggregate ratio , recalcification ( RT ) , and prothrombin time ( PT ) .
	manualset3
127133	5	405629	13	NULL	NULL	0	NULL	activation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged exercise ( 60 min ) performed on a bicycle ergometer in aerobic conditions led to strong activation of the fibrinolytic system ( euglobulin lysis time ( ELT ) fell from 208 to 88 min ) and a slight increase in platelet count ( PC ) but did not cause significant changes in platelet factor 4 ( PF 4 ) and platelet aggregate ratio , recalcification ( RT ) , and prothrombin time ( PT ) .
	manualset3
127134	6	405629	13	NULL	NULL	0	NULL	fibrinolytic system 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged exercise ( 60 min ) performed on a bicycle ergometer in aerobic conditions led to strong activation of the fibrinolytic system ( euglobulin lysis time ( ELT ) fell from 208 to 88 min ) and a slight increase in platelet count ( PC ) but did not cause significant changes in platelet factor 4 ( PF 4 ) and platelet aggregate ratio , recalcification ( RT ) , and prothrombin time ( PT ) .
	manualset3
127135	7	405629	13	NULL	NULL	NULL	NULL	euglobulin lysis time ( ELT ) 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Prolonged exercise ( 60 min ) performed on a bicycle ergometer in aerobic conditions led to strong activation of the fibrinolytic system ( euglobulin lysis time ( ELT ) fell from 208 to 88 min ) and a slight increase in platelet count ( PC ) but did not cause significant changes in platelet factor 4 ( PF 4 ) and platelet aggregate ratio , recalcification ( RT ) , and prothrombin time ( PT ) .
	manualset3
127136	8	405629	13	NULL	NULL	0	NULL	208 to 88 min	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged exercise ( 60 min ) performed on a bicycle ergometer in aerobic conditions led to strong activation of the fibrinolytic system ( euglobulin lysis time ( ELT ) fell from 208 to 88 min ) and a slight increase in platelet count ( PC ) but did not cause significant changes in platelet factor 4 ( PF 4 ) and platelet aggregate ratio , recalcification ( RT ) , and prothrombin time ( PT ) .
	manualset3
127137	9	405629	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged exercise ( 60 min ) performed on a bicycle ergometer in aerobic conditions led to strong activation of the fibrinolytic system ( euglobulin lysis time ( ELT ) fell from 208 to 88 min ) and a slight increase in platelet count ( PC ) but did not cause significant changes in platelet factor 4 ( PF 4 ) and platelet aggregate ratio , recalcification ( RT ) , and prothrombin time ( PT ) .
	manualset3
127138	10	405629	13	NULL	NULL	0	NULL	platelet count ( PC ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged exercise ( 60 min ) performed on a bicycle ergometer in aerobic conditions led to strong activation of the fibrinolytic system ( euglobulin lysis time ( ELT ) fell from 208 to 88 min ) and a slight increase in platelet count ( PC ) but did not cause significant changes in platelet factor 4 ( PF 4 ) and platelet aggregate ratio , recalcification ( RT ) , and prothrombin time ( PT ) .
	manualset3
127139	11	405629	13	NULL	NULL	0	NULL	significant changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged exercise ( 60 min ) performed on a bicycle ergometer in aerobic conditions led to strong activation of the fibrinolytic system ( euglobulin lysis time ( ELT ) fell from 208 to 88 min ) and a slight increase in platelet count ( PC ) but did not cause significant changes in platelet factor 4 ( PF 4 ) and platelet aggregate ratio , recalcification ( RT ) , and prothrombin time ( PT ) .
	manualset3
127140	12	405629	13	NULL	NULL	0	NULL	platelet factor 4 ( PF 4 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged exercise ( 60 min ) performed on a bicycle ergometer in aerobic conditions led to strong activation of the fibrinolytic system ( euglobulin lysis time ( ELT ) fell from 208 to 88 min ) and a slight increase in platelet count ( PC ) but did not cause significant changes in platelet factor 4 ( PF 4 ) and platelet aggregate ratio , recalcification ( RT ) , and prothrombin time ( PT ) .
	manualset3
127141	13	405629	13	NULL	NULL	0	NULL	platelet aggregate ratio 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged exercise ( 60 min ) performed on a bicycle ergometer in aerobic conditions led to strong activation of the fibrinolytic system ( euglobulin lysis time ( ELT ) fell from 208 to 88 min ) and a slight increase in platelet count ( PC ) but did not cause significant changes in platelet factor 4 ( PF 4 ) and platelet aggregate ratio , recalcification ( RT ) , and prothrombin time ( PT ) .
	manualset3
127142	14	405629	13	NULL	NULL	0	NULL	recalcification ( RT )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged exercise ( 60 min ) performed on a bicycle ergometer in aerobic conditions led to strong activation of the fibrinolytic system ( euglobulin lysis time ( ELT ) fell from 208 to 88 min ) and a slight increase in platelet count ( PC ) but did not cause significant changes in platelet factor 4 ( PF 4 ) and platelet aggregate ratio , recalcification ( RT ) , and prothrombin time ( PT ) .
	manualset3
127143	15	405629	13	NULL	NULL	0	NULL	prothrombin time ( PT ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged exercise ( 60 min ) performed on a bicycle ergometer in aerobic conditions led to strong activation of the fibrinolytic system ( euglobulin lysis time ( ELT ) fell from 208 to 88 min ) and a slight increase in platelet count ( PC ) but did not cause significant changes in platelet factor 4 ( PF 4 ) and platelet aggregate ratio , recalcification ( RT ) , and prothrombin time ( PT ) .
	manualset3
127144	1	405630	13	NULL	NULL	0	NULL	treatment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged treatment ( 10 days ) with 4 % w/v Chelex at 4 degrees C reduced the concentration of zinc , strontium , aluminum , copper , manganese , nickel and chromium from 100 to 2.7 , 12.1 , 7.7 , 22.6 , 13.0 , 14.7 and 53.3 % of their original concentrations , respectively .
	manualset3
127145	2	405630	13	NULL	NULL	0	NULL	10 days 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged treatment ( 10 days ) with 4 % w/v Chelex at 4 degrees C reduced the concentration of zinc , strontium , aluminum , copper , manganese , nickel and chromium from 100 to 2.7 , 12.1 , 7.7 , 22.6 , 13.0 , 14.7 and 53.3 % of their original concentrations , respectively .
	manualset3
127146	3	405630	13	NULL	NULL	0	NULL	4 % w/v Chelex 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged treatment ( 10 days ) with 4 % w/v Chelex at 4 degrees C reduced the concentration of zinc , strontium , aluminum , copper , manganese , nickel and chromium from 100 to 2.7 , 12.1 , 7.7 , 22.6 , 13.0 , 14.7 and 53.3 % of their original concentrations , respectively .
	manualset3
127147	4	405630	13	NULL	NULL	0	NULL	4 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged treatment ( 10 days ) with 4 % w/v Chelex at 4 degrees C reduced the concentration of zinc , strontium , aluminum , copper , manganese , nickel and chromium from 100 to 2.7 , 12.1 , 7.7 , 22.6 , 13.0 , 14.7 and 53.3 % of their original concentrations , respectively .
	manualset3
127148	5	405630	13	NULL	NULL	0	NULL	concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged treatment ( 10 days ) with 4 % w/v Chelex at 4 degrees C reduced the concentration of zinc , strontium , aluminum , copper , manganese , nickel and chromium from 100 to 2.7 , 12.1 , 7.7 , 22.6 , 13.0 , 14.7 and 53.3 % of their original concentrations , respectively .
	manualset3
127149	6	405630	13	NULL	NULL	0	NULL	zinc 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged treatment ( 10 days ) with 4 % w/v Chelex at 4 degrees C reduced the concentration of zinc , strontium , aluminum , copper , manganese , nickel and chromium from 100 to 2.7 , 12.1 , 7.7 , 22.6 , 13.0 , 14.7 and 53.3 % of their original concentrations , respectively .
	manualset3
127150	7	405630	13	NULL	NULL	0	NULL	strontium 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged treatment ( 10 days ) with 4 % w/v Chelex at 4 degrees C reduced the concentration of zinc , strontium , aluminum , copper , manganese , nickel and chromium from 100 to 2.7 , 12.1 , 7.7 , 22.6 , 13.0 , 14.7 and 53.3 % of their original concentrations , respectively .
	manualset3
127151	8	405630	13	NULL	NULL	0	NULL	aluminum	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged treatment ( 10 days ) with 4 % w/v Chelex at 4 degrees C reduced the concentration of zinc , strontium , aluminum , copper , manganese , nickel and chromium from 100 to 2.7 , 12.1 , 7.7 , 22.6 , 13.0 , 14.7 and 53.3 % of their original concentrations , respectively .
	manualset3
127152	9	405630	13	NULL	NULL	0	NULL	copper	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged treatment ( 10 days ) with 4 % w/v Chelex at 4 degrees C reduced the concentration of zinc , strontium , aluminum , copper , manganese , nickel and chromium from 100 to 2.7 , 12.1 , 7.7 , 22.6 , 13.0 , 14.7 and 53.3 % of their original concentrations , respectively .
	manualset3
127153	10	405630	13	NULL	NULL	0	NULL	manganese	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged treatment ( 10 days ) with 4 % w/v Chelex at 4 degrees C reduced the concentration of zinc , strontium , aluminum , copper , manganese , nickel and chromium from 100 to 2.7 , 12.1 , 7.7 , 22.6 , 13.0 , 14.7 and 53.3 % of their original concentrations , respectively .
	manualset3
127154	11	405630	13	NULL	NULL	0	NULL	nickel	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged treatment ( 10 days ) with 4 % w/v Chelex at 4 degrees C reduced the concentration of zinc , strontium , aluminum , copper , manganese , nickel and chromium from 100 to 2.7 , 12.1 , 7.7 , 22.6 , 13.0 , 14.7 and 53.3 % of their original concentrations , respectively .
	manualset3
127155	12	405630	13	NULL	NULL	0	NULL	chromium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged treatment ( 10 days ) with 4 % w/v Chelex at 4 degrees C reduced the concentration of zinc , strontium , aluminum , copper , manganese , nickel and chromium from 100 to 2.7 , 12.1 , 7.7 , 22.6 , 13.0 , 14.7 and 53.3 % of their original concentrations , respectively .
	manualset3
127156	13	405630	13	NULL	NULL	0	NULL	100 to 2.7%	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged treatment ( 10 days ) with 4 % w/v Chelex at 4 degrees C reduced the concentration of zinc , strontium , aluminum , copper , manganese , nickel and chromium from 100 to 2.7 , 12.1 , 7.7 , 22.6 , 13.0 , 14.7 and 53.3 % of their original concentrations , respectively .
	manualset3
127157	14	405630	13	NULL	NULL	0	NULL	100 to 12.1%	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged treatment ( 10 days ) with 4 % w/v Chelex at 4 degrees C reduced the concentration of zinc , strontium , aluminum , copper , manganese , nickel and chromium from 100 to 2.7 , 12.1 , 7.7 , 22.6 , 13.0 , 14.7 and 53.3 % of their original concentrations , respectively .
	manualset3
127158	15	405630	13	NULL	NULL	0	NULL	100 to 7.7%	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged treatment ( 10 days ) with 4 % w/v Chelex at 4 degrees C reduced the concentration of zinc , strontium , aluminum , copper , manganese , nickel and chromium from 100 to 2.7 , 12.1 , 7.7 , 22.6 , 13.0 , 14.7 and 53.3 % of their original concentrations , respectively .
	manualset3
127159	16	405630	13	NULL	NULL	0	NULL	100 to 22.6%	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged treatment ( 10 days ) with 4 % w/v Chelex at 4 degrees C reduced the concentration of zinc , strontium , aluminum , copper , manganese , nickel and chromium from 100 to 2.7 , 12.1 , 7.7 , 22.6 , 13.0 , 14.7 and 53.3 % of their original concentrations , respectively .
	manualset3
127160	17	405630	13	NULL	NULL	0	NULL	100 to 13.0%	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged treatment ( 10 days ) with 4 % w/v Chelex at 4 degrees C reduced the concentration of zinc , strontium , aluminum , copper , manganese , nickel and chromium from 100 to 2.7 , 12.1 , 7.7 , 22.6 , 13.0 , 14.7 and 53.3 % of their original concentrations , respectively .
	manualset3
127161	18	405630	13	NULL	NULL	0	NULL	100 to 14.7%	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged treatment ( 10 days ) with 4 % w/v Chelex at 4 degrees C reduced the concentration of zinc , strontium , aluminum , copper , manganese , nickel and chromium from 100 to 2.7 , 12.1 , 7.7 , 22.6 , 13.0 , 14.7 and 53.3 % of their original concentrations , respectively .
	manualset3
127162	19	405630	13	NULL	NULL	0	NULL	100 to 53.3 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged treatment ( 10 days ) with 4 % w/v Chelex at 4 degrees C reduced the concentration of zinc , strontium , aluminum , copper , manganese , nickel and chromium from 100 to 2.7 , 12.1 , 7.7 , 22.6 , 13.0 , 14.7 and 53.3 % of their original concentrations , respectively .
	manualset3
127163	20	405630	13	NULL	NULL	0	NULL	concentrations 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged treatment ( 10 days ) with 4 % w/v Chelex at 4 degrees C reduced the concentration of zinc , strontium , aluminum , copper , manganese , nickel and chromium from 100 to 2.7 , 12.1 , 7.7 , 22.6 , 13.0 , 14.7 and 53.3 % of their original concentrations , respectively .
	manualset3
127164	1	405631	13	NULL	NULL	0	NULL	irradiation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged irradiation leads to the conversion of the ZnO nanosheets into nanorods .
	manualset3
127165	2	405631	13	NULL	NULL	0	NULL	conversion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged irradiation leads to the conversion of the ZnO nanosheets into nanorods .
	manualset3
127166	3	405631	13	NULL	NULL	0	NULL	ZnO nanosheets	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged irradiation leads to the conversion of the ZnO nanosheets into nanorods .
	manualset3
127167	4	405631	13	NULL	NULL	0	NULL	nanorods	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged irradiation leads to the conversion of the ZnO nanosheets into nanorods .
	manualset3
127168	1	405632	13	NULL	NULL	0	NULL	stability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged stability of endogenous cardiotrophin-1 in whole blood .
	manualset3
127169	2	405632	13	NULL	NULL	0	NULL	cardiotrophin-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged stability of endogenous cardiotrophin-1 in whole blood .
	manualset3
127170	3	405632	13	NULL	NULL	0	NULL	blood 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Prolonged stability of endogenous cardiotrophin-1 in whole blood .
	manualset3
127171	1	405633	13	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Promising activity in the MEVM is related to half-lives of NSAID release in plasma , moderate to high lipophilicity , and some degree of inhibition of AChE , a potential contributor to sulfur mustard-mediated tissue damage .
	manualset3
127172	2	405633	13	NULL	NULL	0	NULL	MEVM	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Promising activity in the MEVM is related to half-lives of NSAID release in plasma , moderate to high lipophilicity , and some degree of inhibition of AChE , a potential contributor to sulfur mustard-mediated tissue damage .
	manualset3
127173	3	405633	13	NULL	NULL	0	NULL	half-lives	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Promising activity in the MEVM is related to half-lives of NSAID release in plasma , moderate to high lipophilicity , and some degree of inhibition of AChE , a potential contributor to sulfur mustard-mediated tissue damage .
	manualset3
127174	4	405633	13	NULL	NULL	0	NULL	NSAID release 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Promising activity in the MEVM is related to half-lives of NSAID release in plasma , moderate to high lipophilicity , and some degree of inhibition of AChE , a potential contributor to sulfur mustard-mediated tissue damage .
	manualset3
127175	5	405633	13	NULL	NULL	0	NULL	plasma 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Promising activity in the MEVM is related to half-lives of NSAID release in plasma , moderate to high lipophilicity , and some degree of inhibition of AChE , a potential contributor to sulfur mustard-mediated tissue damage .
	manualset3
127176	6	405633	13	NULL	NULL	0	NULL	lipophilicity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Promising activity in the MEVM is related to half-lives of NSAID release in plasma , moderate to high lipophilicity , and some degree of inhibition of AChE , a potential contributor to sulfur mustard-mediated tissue damage .
	manualset3
127177	7	405633	13	NULL	NULL	0	NULL	degree	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Promising activity in the MEVM is related to half-lives of NSAID release in plasma , moderate to high lipophilicity , and some degree of inhibition of AChE , a potential contributor to sulfur mustard-mediated tissue damage .
	manualset3
127178	8	405633	13	NULL	NULL	0	NULL	inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Promising activity in the MEVM is related to half-lives of NSAID release in plasma , moderate to high lipophilicity , and some degree of inhibition of AChE , a potential contributor to sulfur mustard-mediated tissue damage .
	manualset3
127179	9	405633	13	NULL	NULL	0	NULL	AChE	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Promising activity in the MEVM is related to half-lives of NSAID release in plasma , moderate to high lipophilicity , and some degree of inhibition of AChE , a potential contributor to sulfur mustard-mediated tissue damage .
	manualset3
127180	10	405633	13	NULL	NULL	0	NULL	contributor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Promising activity in the MEVM is related to half-lives of NSAID release in plasma , moderate to high lipophilicity , and some degree of inhibition of AChE , a potential contributor to sulfur mustard-mediated tissue damage .
	manualset3
127181	11	405633	13	NULL	NULL	0	NULL	sulfur mustard-mediated tissue damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Promising activity in the MEVM is related to half-lives of NSAID release in plasma , moderate to high lipophilicity , and some degree of inhibition of AChE , a potential contributor to sulfur mustard-mediated tissue damage .
	manualset3
127182	1	405634	13	NULL	NULL	0	NULL	technologies	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Promising technologies are : the increase of steam parameters , reduction of in-plant energy consumption , and the combined use of heat and power .
	manualset3
127183	2	405634	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Promising technologies are : the increase of steam parameters , reduction of in-plant energy consumption , and the combined use of heat and power .
	manualset3
127184	3	405634	13	NULL	NULL	0	NULL	steam parameters	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Promising technologies are : the increase of steam parameters , reduction of in-plant energy consumption , and the combined use of heat and power .
	manualset3
127185	4	405634	13	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Promising technologies are : the increase of steam parameters , reduction of in-plant energy consumption , and the combined use of heat and power .
	manualset3
127186	5	405634	13	NULL	NULL	0	NULL	energy consumption	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Promising technologies are : the increase of steam parameters , reduction of in-plant energy consumption , and the combined use of heat and power .
	manualset3
127187	6	405634	13	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Promising technologies are : the increase of steam parameters , reduction of in-plant energy consumption , and the combined use of heat and power .
	manualset3
127189	8	405634	13	NULL	NULL	NULL	NULL	heat and power	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Promising technologies are : the increase of steam parameters , reduction of in-plant energy consumption , and the combined use of heat and power .
	manualset3
127190	1	405635	13	NULL	NULL	0	NULL	Promoter activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter activity in myocytes required a single muscle CAT ( MCAT ) element , and this MCAT bound in vitro to recombinant and endogenous transcriptional enhancer factor-1 .
	manualset3
127191	2	405635	13	NULL	NULL	0	NULL	myocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter activity in myocytes required a single muscle CAT ( MCAT ) element , and this MCAT bound in vitro to recombinant and endogenous transcriptional enhancer factor-1 .
	manualset3
127192	3	405635	13	NULL	NULL	0	NULL	muscle CAT ( MCAT ) element	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter activity in myocytes required a single muscle CAT ( MCAT ) element , and this MCAT bound in vitro to recombinant and endogenous transcriptional enhancer factor-1 .
	manualset3
127193	4	405635	13	NULL	NULL	0	NULL	MCAT	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter activity in myocytes required a single muscle CAT ( MCAT ) element , and this MCAT bound in vitro to recombinant and endogenous transcriptional enhancer factor-1 .
	manualset3
127194	5	405635	13	NULL	NULL	0	NULL	transcriptional enhancer factor-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter activity in myocytes required a single muscle CAT ( MCAT ) element , and this MCAT bound in vitro to recombinant and endogenous transcriptional enhancer factor-1 .
	manualset3
127195	1	405636	13	NULL	NULL	0	NULL	Promoter activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter activity was strongly inhibited in a dose-dependent fashion by phorbol ester , with responsiveness mapped to bp -208 / -54 , but was not responsive to glucocorticoid .
	manualset3
127196	2	405636	13	NULL	NULL	0	NULL	 dose-dependent fashion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter activity was strongly inhibited in a dose-dependent fashion by phorbol ester , with responsiveness mapped to bp -208 / -54 , but was not responsive to glucocorticoid .
	manualset3
127197	3	405636	13	NULL	NULL	0	NULL	phorbol ester	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter activity was strongly inhibited in a dose-dependent fashion by phorbol ester , with responsiveness mapped to bp -208 / -54 , but was not responsive to glucocorticoid .
	manualset3
127198	4	405636	13	NULL	NULL	0	NULL	responsiveness	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter activity was strongly inhibited in a dose-dependent fashion by phorbol ester , with responsiveness mapped to bp -208 / -54 , but was not responsive to glucocorticoid .
	manualset3
127199	5	405636	13	NULL	NULL	0	NULL	bp -208 / -54 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter activity was strongly inhibited in a dose-dependent fashion by phorbol ester , with responsiveness mapped to bp -208 / -54 , but was not responsive to glucocorticoid .
	manualset3
127200	6	405636	13	NULL	NULL	0	NULL	glucocorticoid	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter activity was strongly inhibited in a dose-dependent fashion by phorbol ester , with responsiveness mapped to bp -208 / -54 , but was not responsive to glucocorticoid .
	manualset3
127201	1	405637	13	NULL	NULL	0	NULL	Promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter hypermethylation in 10 tumor-related genes ( APC , ATM , GSTP1 , HLTF , MGMT , hMLH1 , p14 , p15 , SOCS-1 and TIMP-3 ) were studied by methylation-specific PCR .
	manualset3
127202	2	405637	13	NULL	NULL	0	NULL	hypermethylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter hypermethylation in 10 tumor-related genes ( APC , ATM , GSTP1 , HLTF , MGMT , hMLH1 , p14 , p15 , SOCS-1 and TIMP-3 ) were studied by methylation-specific PCR .
	manualset3
127203	3	405637	13	NULL	NULL	0	NULL	10 tumor-related genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter hypermethylation in 10 tumor-related genes ( APC , ATM , GSTP1 , HLTF , MGMT , hMLH1 , p14 , p15 , SOCS-1 and TIMP-3 ) were studied by methylation-specific PCR .
	manualset3
127204	4	405637	13	NULL	NULL	0	NULL	APC	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter hypermethylation in 10 tumor-related genes ( APC , ATM , GSTP1 , HLTF , MGMT , hMLH1 , p14 , p15 , SOCS-1 and TIMP-3 ) were studied by methylation-specific PCR .
	manualset3
127205	5	405637	13	NULL	NULL	0	NULL	ATM	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter hypermethylation in 10 tumor-related genes ( APC , ATM , GSTP1 , HLTF , MGMT , hMLH1 , p14 , p15 , SOCS-1 and TIMP-3 ) were studied by methylation-specific PCR .
	manualset3
127206	6	405637	13	NULL	NULL	0	NULL	GSTP1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter hypermethylation in 10 tumor-related genes ( APC , ATM , GSTP1 , HLTF , MGMT , hMLH1 , p14 , p15 , SOCS-1 and TIMP-3 ) were studied by methylation-specific PCR .
	manualset3
127207	7	405637	13	NULL	NULL	0	NULL	HLTF	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter hypermethylation in 10 tumor-related genes ( APC , ATM , GSTP1 , HLTF , MGMT , hMLH1 , p14 , p15 , SOCS-1 and TIMP-3 ) were studied by methylation-specific PCR .
	manualset3
127208	8	405637	13	NULL	NULL	0	NULL	MGMT	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter hypermethylation in 10 tumor-related genes ( APC , ATM , GSTP1 , HLTF , MGMT , hMLH1 , p14 , p15 , SOCS-1 and TIMP-3 ) were studied by methylation-specific PCR .
	manualset3
127209	9	405637	13	NULL	NULL	0	NULL	hMLH1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter hypermethylation in 10 tumor-related genes ( APC , ATM , GSTP1 , HLTF , MGMT , hMLH1 , p14 , p15 , SOCS-1 and TIMP-3 ) were studied by methylation-specific PCR .
	manualset3
127210	10	405637	13	NULL	NULL	0	NULL	p14 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter hypermethylation in 10 tumor-related genes ( APC , ATM , GSTP1 , HLTF , MGMT , hMLH1 , p14 , p15 , SOCS-1 and TIMP-3 ) were studied by methylation-specific PCR .
	manualset3
127211	11	405637	13	NULL	NULL	0	NULL	p15	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter hypermethylation in 10 tumor-related genes ( APC , ATM , GSTP1 , HLTF , MGMT , hMLH1 , p14 , p15 , SOCS-1 and TIMP-3 ) were studied by methylation-specific PCR .
	manualset3
127212	12	405637	13	NULL	NULL	0	NULL	SOCS-1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter hypermethylation in 10 tumor-related genes ( APC , ATM , GSTP1 , HLTF , MGMT , hMLH1 , p14 , p15 , SOCS-1 and TIMP-3 ) were studied by methylation-specific PCR .
	manualset3
127213	13	405637	13	NULL	NULL	0	NULL	TIMP-3	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter hypermethylation in 10 tumor-related genes ( APC , ATM , GSTP1 , HLTF , MGMT , hMLH1 , p14 , p15 , SOCS-1 and TIMP-3 ) were studied by methylation-specific PCR .
	manualset3
127214	14	405637	13	NULL	NULL	0	NULL	methylation-specific PCR 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Promoter hypermethylation in 10 tumor-related genes ( APC , ATM , GSTP1 , HLTF , MGMT , hMLH1 , p14 , p15 , SOCS-1 and TIMP-3 ) were studied by methylation-specific PCR .
	manualset3
127215	1	405638	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prompt differential diagnosis between the subsets is critical , because therapeutic strategy may differ in the use of high-dose corticosteroid and plasma exchange between the subsets of PRS .
	manualset3
127216	2	405638	13	NULL	NULL	0	NULL	subsets	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Prompt differential diagnosis between the subsets is critical , because therapeutic strategy may differ in the use of high-dose corticosteroid and plasma exchange between the subsets of PRS .
	manualset3
127217	3	405638	13	NULL	NULL	0	NULL	therapeutic strategy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prompt differential diagnosis between the subsets is critical , because therapeutic strategy may differ in the use of high-dose corticosteroid and plasma exchange between the subsets of PRS .
	manualset3
127218	4	405638	13	NULL	NULL	0	NULL	high-dose corticosteroid 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prompt differential diagnosis between the subsets is critical , because therapeutic strategy may differ in the use of high-dose corticosteroid and plasma exchange between the subsets of PRS .
	manualset3
127219	5	405638	13	NULL	NULL	0	NULL	plasma exchange	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Prompt differential diagnosis between the subsets is critical , because therapeutic strategy may differ in the use of high-dose corticosteroid and plasma exchange between the subsets of PRS .
	manualset3
127220	6	405638	13	NULL	NULL	0	NULL	subsets	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Prompt differential diagnosis between the subsets is critical , because therapeutic strategy may differ in the use of high-dose corticosteroid and plasma exchange between the subsets of PRS .
	manualset3
127221	7	405638	13	NULL	NULL	0	NULL	PRS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Prompt differential diagnosis between the subsets is critical , because therapeutic strategy may differ in the use of high-dose corticosteroid and plasma exchange between the subsets of PRS .
	manualset3
127222	1	405639	13	NULL	NULL	0	NULL	initiation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prompt initiation of proper treatment is important for improved outcomes .
	manualset3
127223	2	405639	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prompt initiation of proper treatment is important for improved outcomes .
	manualset3
127224	3	405639	13	NULL	NULL	0	NULL	outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prompt initiation of proper treatment is important for improved outcomes .
	manualset3
127225	1	405640	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prompt diagnosis , resuscitation and early radical surgery are essential to the successful management of necrotizing fasciitis .
	manualset3
127226	2	405640	13	NULL	NULL	0	NULL	resuscitation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prompt diagnosis , resuscitation and early radical surgery are essential to the successful management of necrotizing fasciitis .
	manualset3
127227	3	405640	13	NULL	NULL	0	NULL	radical surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prompt diagnosis , resuscitation and early radical surgery are essential to the successful management of necrotizing fasciitis .
	manualset3
127228	4	405640	13	NULL	NULL	0	NULL	management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prompt diagnosis , resuscitation and early radical surgery are essential to the successful management of necrotizing fasciitis .
	manualset3
127229	5	405640	13	NULL	NULL	0	NULL	necrotizing fasciitis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prompt diagnosis , resuscitation and early radical surgery are essential to the successful management of necrotizing fasciitis .
	manualset3
127230	1	405641	13	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prompt diagnosis is often essential and may even be lifesaving .
	manualset3
127231	1	405642	13	NULL	NULL	0	NULL	position 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prone position as a life-saving measure for acute pulmonary hemorrhage in a young adult with cystic fibrosis .
	manualset3
127232	2	405642	13	NULL	NULL	0	NULL	life-saving measure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prone position as a life-saving measure for acute pulmonary hemorrhage in a young adult with cystic fibrosis .
	manualset3
127233	3	405642	13	NULL	NULL	0	NULL	acute pulmonary hemorrhage 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prone position as a life-saving measure for acute pulmonary hemorrhage in a young adult with cystic fibrosis .
	manualset3
127234	4	405642	13	NULL	NULL	0	NULL	young adult	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Prone position as a life-saving measure for acute pulmonary hemorrhage in a young adult with cystic fibrosis .
	manualset3
127235	5	405642	13	NULL	NULL	0	NULL	cystic fibrosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Prone position as a life-saving measure for acute pulmonary hemorrhage in a young adult with cystic fibrosis .
	manualset3
127236	1	405643	13	NULL	NULL	0	NULL	adoption 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Proper adoption of the new technology will require a new quantitative mentality in pathology .
	manualset3
127237	2	405643	13	NULL	NULL	0	NULL	new technology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Proper adoption of the new technology will require a new quantitative mentality in pathology .
	manualset3
127238	3	405643	13	NULL	NULL	0	NULL	quantitative mentality 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Proper adoption of the new technology will require a new quantitative mentality in pathology .
	manualset3
127239	4	405643	13	NULL	NULL	0	NULL	pathology 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Proper adoption of the new technology will require a new quantitative mentality in pathology .
	manualset3
127240	1	405644	13	NULL	NULL	0	NULL	physical planning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Proper physical and social planning ; knowledge of the geography , entomology , epidemiology , behavior , and life-cycle of the malaria parasite ; and official and international cooperation are needed to control and eradicate malaria in this setting .
	manualset3
127241	2	405644	13	NULL	NULL	0	NULL	social planning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Proper physical and social planning ; knowledge of the geography , entomology , epidemiology , behavior , and life-cycle of the malaria parasite ; and official and international cooperation are needed to control and eradicate malaria in this setting .
	manualset3
127242	3	405644	13	NULL	NULL	0	NULL	knowledge	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Proper physical and social planning ; knowledge of the geography , entomology , epidemiology , behavior , and life-cycle of the malaria parasite ; and official and international cooperation are needed to control and eradicate malaria in this setting .
	manualset3
127243	4	405644	13	NULL	NULL	NULL	NULL	geography	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Proper physical and social planning ; knowledge of the geography , entomology , epidemiology , behavior , and life-cycle of the malaria parasite ; and official and international cooperation are needed to control and eradicate malaria in this setting .
	manualset3
127244	5	405644	13	NULL	NULL	NULL	NULL	entomology	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Proper physical and social planning ; knowledge of the geography , entomology , epidemiology , behavior , and life-cycle of the malaria parasite ; and official and international cooperation are needed to control and eradicate malaria in this setting .
	manualset3
127245	6	405644	13	NULL	NULL	0	NULL	epidemiology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Proper physical and social planning ; knowledge of the geography , entomology , epidemiology , behavior , and life-cycle of the malaria parasite ; and official and international cooperation are needed to control and eradicate malaria in this setting .
	manualset3
127246	7	405644	13	NULL	NULL	0	NULL	behavior	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Proper physical and social planning ; knowledge of the geography , entomology , epidemiology , behavior , and life-cycle of the malaria parasite ; and official and international cooperation are needed to control and eradicate malaria in this setting .
	manualset3
127247	8	405644	13	NULL	NULL	0	NULL	life-cycle	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Proper physical and social planning ; knowledge of the geography , entomology , epidemiology , behavior , and life-cycle of the malaria parasite ; and official and international cooperation are needed to control and eradicate malaria in this setting .
	manualset3
127248	9	405644	13	NULL	NULL	0	NULL	malaria parasite	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Proper physical and social planning ; knowledge of the geography , entomology , epidemiology , behavior , and life-cycle of the malaria parasite ; and official and international cooperation are needed to control and eradicate malaria in this setting .
	manualset3
127249	10	405644	13	NULL	NULL	0	NULL	official cooperation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Proper physical and social planning ; knowledge of the geography , entomology , epidemiology , behavior , and life-cycle of the malaria parasite ; and official and international cooperation are needed to control and eradicate malaria in this setting .
	manualset3
127250	11	405644	13	NULL	NULL	0	NULL	international cooperation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Proper physical and social planning ; knowledge of the geography , entomology , epidemiology , behavior , and life-cycle of the malaria parasite ; and official and international cooperation are needed to control and eradicate malaria in this setting .
	manualset3
127251	12	405644	13	NULL	NULL	0	NULL	malaria	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Proper physical and social planning ; knowledge of the geography , entomology , epidemiology , behavior , and life-cycle of the malaria parasite ; and official and international cooperation are needed to control and eradicate malaria in this setting .
	manualset3
127252	13	405644	13	NULL	NULL	0	NULL	setting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Proper physical and social planning ; knowledge of the geography , entomology , epidemiology , behavior , and life-cycle of the malaria parasite ; and official and international cooperation are needed to control and eradicate malaria in this setting .
	manualset3
127253	1	405645	13	NULL	NULL	0	NULL	Properties	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Properties of Sindbis virus vectors produced with a chimeric split helper system .
	manualset3
127254	2	405645	13	NULL	NULL	0	NULL	Sindbis virus vectors	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Properties of Sindbis virus vectors produced with a chimeric split helper system .
	manualset3
127255	3	405645	13	NULL	NULL	0	NULL	chimeric split helper system 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Properties of Sindbis virus vectors produced with a chimeric split helper system .
	manualset3
127256	1	405646	13	NULL	NULL	0	NULL	Properties	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Properties of a phenolase preparation from cell suspension cultures of parsley .
	manualset3
127257	2	405646	13	NULL	NULL	0	NULL	phenolase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Properties of a phenolase preparation from cell suspension cultures of parsley .
	manualset3
127258	3	405646	13	NULL	NULL	0	NULL	preparation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Properties of a phenolase preparation from cell suspension cultures of parsley .
	manualset3
127259	4	405646	13	NULL	NULL	0	NULL	cell suspension cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Properties of a phenolase preparation from cell suspension cultures of parsley .
	manualset3
127260	5	405646	13	NULL	NULL	0	NULL	parsley	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Properties of a phenolase preparation from cell suspension cultures of parsley .
	manualset3
127261	1	405647	13	NULL	NULL	0	NULL	Properties	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Properties of horse liver alcohol dehydrogenase modified by the affinity label 3-chloroacetylpyridine-adenine dinucleotide .
	manualset3
127262	2	405647	13	NULL	NULL	0	NULL	horse liver alcohol dehydrogenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Properties of horse liver alcohol dehydrogenase modified by the affinity label 3-chloroacetylpyridine-adenine dinucleotide .
	manualset3
127263	3	405647	13	NULL	NULL	0	NULL	affinity label 3-chloroacetylpyridine-adenine dinucleotide	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Properties of horse liver alcohol dehydrogenase modified by the affinity label 3-chloroacetylpyridine-adenine dinucleotide .
	manualset3
127264	1	405648	13	NULL	NULL	0	NULL	Properties	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Properties of sarcolemmal delayed rectification in glycerol-treated fibers of frog sartorius muscle .
	manualset3
127265	2	405648	13	NULL	NULL	0	NULL	sarcolemmal	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Properties of sarcolemmal delayed rectification in glycerol-treated fibers of frog sartorius muscle .
	manualset3
127266	3	405648	13	NULL	NULL	0	NULL	rectification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Properties of sarcolemmal delayed rectification in glycerol-treated fibers of frog sartorius muscle .
	manualset3
127267	4	405648	13	NULL	NULL	0	NULL	glycerol-treated fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Properties of sarcolemmal delayed rectification in glycerol-treated fibers of frog sartorius muscle .
	manualset3
127268	5	405648	13	NULL	NULL	0	NULL	frog sartorius muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Properties of sarcolemmal delayed rectification in glycerol-treated fibers of frog sartorius muscle .
	manualset3
127269	1	405649	13	NULL	NULL	0	NULL	Properties	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Properties of the thalamic projection from the posterior medial nucleus to primary and secondary somatosensory cortices in the mouse .
	manualset3
127270	2	405649	13	NULL	NULL	0	NULL	thalamic projection	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Properties of the thalamic projection from the posterior medial nucleus to primary and secondary somatosensory cortices in the mouse .
	manualset3
127271	3	405649	13	NULL	NULL	0	NULL	posterior medial nucleus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Properties of the thalamic projection from the posterior medial nucleus to primary and secondary somatosensory cortices in the mouse .
	manualset3
127272	4	405649	13	NULL	NULL	0	NULL	primary somatosensory cortices	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Properties of the thalamic projection from the posterior medial nucleus to primary and secondary somatosensory cortices in the mouse .
	manualset3
127273	5	405649	13	NULL	NULL	0	NULL	secondary somatosensory cortices 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Properties of the thalamic projection from the posterior medial nucleus to primary and secondary somatosensory cortices in the mouse .
	manualset3
127274	6	405649	13	NULL	NULL	0	NULL	mouse	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Properties of the thalamic projection from the posterior medial nucleus to primary and secondary somatosensory cortices in the mouse .
	manualset3
127275	1	405650	13	NULL	NULL	0	NULL	magnetic measurement device	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A magnetic measurement device is described which was constructed to study human hand - and finger-movements .
	manualset3
127276	2	405650	13	NULL	NULL	0	NULL	human hand -movements	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A magnetic measurement device is described which was constructed to study human hand - and finger-movements .
	manualset3
127277	3	405650	13	NULL	NULL	0	NULL	human finger-movements 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A magnetic measurement device is described which was constructed to study human hand - and finger-movements .
	manualset3
127278	1	405651	13	NULL	NULL	0	NULL	Prophylactic topical acyclovir	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Prophylactic topical acyclovir for frequent recurrent herpes simplex infection with and without erythema multiforme .
	manualset3
127279	2	405651	13	NULL	NULL	0	NULL	recurrent herpes simplex infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prophylactic topical acyclovir for frequent recurrent herpes simplex infection with and without erythema multiforme .
	manualset3
127280	3	405651	13	NULL	NULL	0	NULL	erythema multiforme	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prophylactic topical acyclovir for frequent recurrent herpes simplex infection with and without erythema multiforme .
	manualset3
127281	1	405652	13	NULL	NULL	0	NULL	Prophylaxis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prophylaxis of dysrhythmias after myocardial infarction .
	manualset3
127282	2	405652	13	NULL	NULL	0	NULL	dysrhythmias 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prophylaxis of dysrhythmias after myocardial infarction .
	manualset3
127283	3	405652	13	NULL	NULL	0	NULL	myocardial infarction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prophylaxis of dysrhythmias after myocardial infarction .
	manualset3
127284	1	405653	13	NULL	NULL	0	NULL	Propofol 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Propofol pretreatment reduces ceramide production and attenuates intestinal mucosal apoptosis induced by intestinal ischemia/reperfusion in rats .
	manualset3
127285	2	405653	13	NULL	NULL	0	NULL	pretreatment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Propofol pretreatment reduces ceramide production and attenuates intestinal mucosal apoptosis induced by intestinal ischemia/reperfusion in rats .
	manualset3
127286	3	405653	13	NULL	NULL	0	NULL	ceramide 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Propofol pretreatment reduces ceramide production and attenuates intestinal mucosal apoptosis induced by intestinal ischemia/reperfusion in rats .
	manualset3
127287	4	405653	13	NULL	NULL	0	NULL	production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Propofol pretreatment reduces ceramide production and attenuates intestinal mucosal apoptosis induced by intestinal ischemia/reperfusion in rats .
	manualset3
127288	5	405653	13	NULL	NULL	0	NULL	intestinal mucosal apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Propofol pretreatment reduces ceramide production and attenuates intestinal mucosal apoptosis induced by intestinal ischemia/reperfusion in rats .
	manualset3
127289	6	405653	13	NULL	NULL	0	NULL	intestinal ischemia/reperfusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Propofol pretreatment reduces ceramide production and attenuates intestinal mucosal apoptosis induced by intestinal ischemia/reperfusion in rats .
	manualset3
127290	7	405653	13	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Propofol pretreatment reduces ceramide production and attenuates intestinal mucosal apoptosis induced by intestinal ischemia/reperfusion in rats .
	manualset3
127291	1	405654	13	NULL	NULL	0	NULL	Proposal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Proposal for classifying the acute emetogenicity of cancer chemotherapy .
	manualset3
127292	2	405654	13	NULL	NULL	0	NULL	acute emetogenicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Proposal for classifying the acute emetogenicity of cancer chemotherapy .
	manualset3
127293	3	405654	13	NULL	NULL	0	NULL	cancer chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Proposal for classifying the acute emetogenicity of cancer chemotherapy .
	manualset3
127294	1	405655	13	NULL	NULL	0	NULL	Prosodic deficits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prosodic deficits characterize a subset of individuals with schizotypy who show a schizoid-like reduction in social behaviors without a concomitant reduction in social satisfaction .
	manualset3
127295	2	405655	13	NULL	NULL	0	NULL	subset of individuals 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Prosodic deficits characterize a subset of individuals with schizotypy who show a schizoid-like reduction in social behaviors without a concomitant reduction in social satisfaction .
	manualset3
127296	3	405655	13	NULL	NULL	0	NULL	schizotypy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prosodic deficits characterize a subset of individuals with schizotypy who show a schizoid-like reduction in social behaviors without a concomitant reduction in social satisfaction .
	manualset3
127297	4	405655	13	NULL	NULL	0	NULL	schizoid-like reduction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prosodic deficits characterize a subset of individuals with schizotypy who show a schizoid-like reduction in social behaviors without a concomitant reduction in social satisfaction .
	manualset3
127298	5	405655	13	NULL	NULL	0	NULL	social behaviors	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prosodic deficits characterize a subset of individuals with schizotypy who show a schizoid-like reduction in social behaviors without a concomitant reduction in social satisfaction .
	manualset3
127299	6	405655	13	NULL	NULL	NULL	NULL	concomitant reduction	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Prosodic deficits characterize a subset of individuals with schizotypy who show a schizoid-like reduction in social behaviors without a concomitant reduction in social satisfaction .
	manualset3
127300	7	405655	13	NULL	NULL	0	NULL	social satisfaction	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Prosodic deficits characterize a subset of individuals with schizotypy who show a schizoid-like reduction in social behaviors without a concomitant reduction in social satisfaction .
	manualset3
127301	1	405656	13	NULL	NULL	0	NULL	amputation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A major amputation had been indicated because the infection did not respond to antibiotics and advanced wound care with topical negative pressure wound therapy with silver .
	manualset3
127302	2	405656	13	NULL	NULL	0	NULL	infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A major amputation had been indicated because the infection did not respond to antibiotics and advanced wound care with topical negative pressure wound therapy with silver .
	manualset3
127303	3	405656	13	NULL	NULL	0	NULL	antibiotics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A major amputation had been indicated because the infection did not respond to antibiotics and advanced wound care with topical negative pressure wound therapy with silver .
	manualset3
127304	4	405656	13	NULL	NULL	0	NULL	wound care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A major amputation had been indicated because the infection did not respond to antibiotics and advanced wound care with topical negative pressure wound therapy with silver .
	manualset3
127305	5	405656	13	NULL	NULL	0	NULL	topical negative pressure wound therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A major amputation had been indicated because the infection did not respond to antibiotics and advanced wound care with topical negative pressure wound therapy with silver .
	manualset3
127306	6	405656	13	NULL	NULL	0	NULL	silver 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	A major amputation had been indicated because the infection did not respond to antibiotics and advanced wound care with topical negative pressure wound therapy with silver .
	manualset3
127307	1	405657	13	NULL	NULL	0	NULL	Prospective evaluation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prospective evaluation by computed tomography and pulmonary function tests of children with mediastinal masses .
	manualset3
127308	2	405657	13	NULL	NULL	0	NULL	computed tomography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prospective evaluation by computed tomography and pulmonary function tests of children with mediastinal masses .
	manualset3
127309	3	405657	13	NULL	NULL	0	NULL	pulmonary function tests	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prospective evaluation by computed tomography and pulmonary function tests of children with mediastinal masses .
	manualset3
127310	4	405657	13	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Prospective evaluation by computed tomography and pulmonary function tests of children with mediastinal masses .
	manualset3
127311	5	405657	13	NULL	NULL	0	NULL	mediastinal masses 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prospective evaluation by computed tomography and pulmonary function tests of children with mediastinal masses .
	manualset3
127312	1	405658	13	NULL	NULL	0	NULL	Prospective evaluation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prospective evaluation of concomitant lymphadenectomy in robot-assisted radical prostatectomy : preliminary analysis of outcomes .
	manualset3
127313	2	405658	13	NULL	NULL	0	NULL	concomitant lymphadenectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prospective evaluation of concomitant lymphadenectomy in robot-assisted radical prostatectomy : preliminary analysis of outcomes .
	manualset3
127314	3	405658	13	NULL	NULL	0	NULL	robot-assisted radical prostatectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prospective evaluation of concomitant lymphadenectomy in robot-assisted radical prostatectomy : preliminary analysis of outcomes .
	manualset3
127315	4	405658	13	NULL	NULL	0	NULL	preliminary analysis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prospective evaluation of concomitant lymphadenectomy in robot-assisted radical prostatectomy : preliminary analysis of outcomes .
	manualset3
127316	5	405658	13	NULL	NULL	0	NULL	outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prospective evaluation of concomitant lymphadenectomy in robot-assisted radical prostatectomy : preliminary analysis of outcomes .
	manualset3
127317	1	405659	13	NULL	NULL	0	NULL	randomized trials	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Prospective randomized trials are needed to evaluate this approach as compared with RT alone and to define its precise role in locally advanced cervical cancer .
	manualset3
127318	2	405659	13	NULL	NULL	0	NULL	approach	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Prospective randomized trials are needed to evaluate this approach as compared with RT alone and to define its precise role in locally advanced cervical cancer .
	manualset3
127319	3	405659	13	NULL	NULL	0	NULL	RT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prospective randomized trials are needed to evaluate this approach as compared with RT alone and to define its precise role in locally advanced cervical cancer .
	manualset3
127320	4	405659	13	NULL	NULL	0	NULL	cervical cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Prospective randomized trials are needed to evaluate this approach as compared with RT alone and to define its precise role in locally advanced cervical cancer .
	manualset3
128815	5	405659	13	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prospective randomized trials are needed to evaluate this approach as compared with RT alone and to define its precise role in locally advanced cervical cancer .
	manualset3
127321	1	405660	13	NULL	NULL	0	NULL	Prostacyclin ( PGI2 ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Prostacyclin ( PGI2 ) is the major cyclo oxygenase metabolite in the rat gastric mucosa and exerts gastroprotective actions .
	manualset3
127322	2	405660	13	NULL	NULL	0	NULL	major cyclo oxygenase metabolite 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Prostacyclin ( PGI2 ) is the major cyclo oxygenase metabolite in the rat gastric mucosa and exerts gastroprotective actions .
	manualset3
127323	3	405660	13	NULL	NULL	0	NULL	rat gastric mucosa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Prostacyclin ( PGI2 ) is the major cyclo oxygenase metabolite in the rat gastric mucosa and exerts gastroprotective actions .
	manualset3
127324	4	405660	13	NULL	NULL	0	NULL	gastroprotective actions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prostacyclin ( PGI2 ) is the major cyclo oxygenase metabolite in the rat gastric mucosa and exerts gastroprotective actions .
	manualset3
127325	1	405661	13	NULL	NULL	0	NULL	Prostaglandins	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Prostaglandins were the major metabolites from extracellular arachidonic acid .
	manualset3
127326	2	405661	13	NULL	NULL	0	NULL	major metabolites	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Prostaglandins were the major metabolites from extracellular arachidonic acid .
	manualset3
127327	3	405661	13	NULL	NULL	0	NULL	extracellular arachidonic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Prostaglandins were the major metabolites from extracellular arachidonic acid .
	manualset3
127328	1	405662	13	NULL	NULL	0	NULL	Prostate specific antigen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Prostate specific antigen in urinary tract infection .
	manualset3
127329	2	405662	13	NULL	NULL	0	NULL	urinary tract infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prostate specific antigen in urinary tract infection .
	manualset3
127330	1	405663	13	NULL	NULL	0	NULL	Protagonist	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Protagonist : population based endoscopic screening for colorectal cancer .
	manualset3
127331	2	405663	13	NULL	NULL	0	NULL	population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Protagonist : population based endoscopic screening for colorectal cancer .
	manualset3
127332	3	405663	13	NULL	NULL	0	NULL	endoscopic screening	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Protagonist : population based endoscopic screening for colorectal cancer .
	manualset3
127333	4	405663	13	NULL	NULL	0	NULL	colorectal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Protagonist : population based endoscopic screening for colorectal cancer .
	manualset3
127334	1	405664	13	NULL	NULL	0	NULL	cell-binding domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A major cell-binding domain was found to reside near the intersection point of the short arms , and the type IV collagen-binding domain was associated with the globular end regions of the short arms .
	manualset3
127335	2	405664	13	NULL	NULL	0	NULL	 intersection point	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A major cell-binding domain was found to reside near the intersection point of the short arms , and the type IV collagen-binding domain was associated with the globular end regions of the short arms .
	manualset3
127336	3	405664	13	NULL	NULL	0	NULL	short arms	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A major cell-binding domain was found to reside near the intersection point of the short arms , and the type IV collagen-binding domain was associated with the globular end regions of the short arms .
	manualset3
127337	4	405664	13	NULL	NULL	0	NULL	type IV collagen-binding domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A major cell-binding domain was found to reside near the intersection point of the short arms , and the type IV collagen-binding domain was associated with the globular end regions of the short arms .
	manualset3
127338	5	405664	13	NULL	NULL	0	NULL	globular end regions 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A major cell-binding domain was found to reside near the intersection point of the short arms , and the type IV collagen-binding domain was associated with the globular end regions of the short arms .
	manualset3
127339	6	405664	13	NULL	NULL	0	NULL	short arms	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A major cell-binding domain was found to reside near the intersection point of the short arms , and the type IV collagen-binding domain was associated with the globular end regions of the short arms .
	manualset3
127340	1	405665	13	NULL	NULL	0	NULL	Protamine	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Protamine depressed mean ( s.d. ) myocardial left ventricular pressure in both non-ischaemic hearts ( groups 2 and 3 , to 49 ( 4 ) % and 50 ( 4 ) % from baseline , respectively ) and post ischaemic hearts ( group 5 , to 28 ( 8 % ) .
	manualset3
127341	2	405665	13	NULL	NULL	0	NULL	mean ( s.d. ) myocardial left ventricular pressure 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Protamine depressed mean ( s.d. ) myocardial left ventricular pressure in both non-ischaemic hearts ( groups 2 and 3 , to 49 ( 4 ) % and 50 ( 4 ) % from baseline , respectively ) and post ischaemic hearts ( group 5 , to 28 ( 8 % ) .
	manualset3
127342	3	405665	13	NULL	NULL	0	NULL	non-ischaemic hearts 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Protamine depressed mean ( s.d. ) myocardial left ventricular pressure in both non-ischaemic hearts ( groups 2 and 3 , to 49 ( 4 ) % and 50 ( 4 ) % from baseline , respectively ) and post ischaemic hearts ( group 5 , to 28 ( 8 % ) .
	manualset3
127343	4	405665	13	NULL	NULL	0	NULL	groups 2	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Protamine depressed mean ( s.d. ) myocardial left ventricular pressure in both non-ischaemic hearts ( groups 2 and 3 , to 49 ( 4 ) % and 50 ( 4 ) % from baseline , respectively ) and post ischaemic hearts ( group 5 , to 28 ( 8 % ) .
	manualset3
127344	5	405665	13	NULL	NULL	0	NULL	groups 3	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Protamine depressed mean ( s.d. ) myocardial left ventricular pressure in both non-ischaemic hearts ( groups 2 and 3 , to 49 ( 4 ) % and 50 ( 4 ) % from baseline , respectively ) and post ischaemic hearts ( group 5 , to 28 ( 8 % ) .
	manualset3
127345	6	405665	13	NULL	NULL	0	NULL	49 ( 4 ) % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Protamine depressed mean ( s.d. ) myocardial left ventricular pressure in both non-ischaemic hearts ( groups 2 and 3 , to 49 ( 4 ) % and 50 ( 4 ) % from baseline , respectively ) and post ischaemic hearts ( group 5 , to 28 ( 8 % ) .
	manualset3
127346	7	405665	13	NULL	NULL	0	NULL	50 ( 4 ) %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Protamine depressed mean ( s.d. ) myocardial left ventricular pressure in both non-ischaemic hearts ( groups 2 and 3 , to 49 ( 4 ) % and 50 ( 4 ) % from baseline , respectively ) and post ischaemic hearts ( group 5 , to 28 ( 8 % ) .
	manualset3
127347	8	405665	13	NULL	NULL	0	NULL	baseline	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Protamine depressed mean ( s.d. ) myocardial left ventricular pressure in both non-ischaemic hearts ( groups 2 and 3 , to 49 ( 4 ) % and 50 ( 4 ) % from baseline , respectively ) and post ischaemic hearts ( group 5 , to 28 ( 8 % ) .
	manualset3
127348	9	405665	13	NULL	NULL	0	NULL	post ischaemic hearts 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Protamine depressed mean ( s.d. ) myocardial left ventricular pressure in both non-ischaemic hearts ( groups 2 and 3 , to 49 ( 4 ) % and 50 ( 4 ) % from baseline , respectively ) and post ischaemic hearts ( group 5 , to 28 ( 8 % ) .
	manualset3
127349	10	405665	13	NULL	NULL	0	NULL	group 5	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Protamine depressed mean ( s.d. ) myocardial left ventricular pressure in both non-ischaemic hearts ( groups 2 and 3 , to 49 ( 4 ) % and 50 ( 4 ) % from baseline , respectively ) and post ischaemic hearts ( group 5 , to 28 ( 8 % ) .
	manualset3
127350	11	405665	13	NULL	NULL	0	NULL	28 ( 8 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Protamine depressed mean ( s.d. ) myocardial left ventricular pressure in both non-ischaemic hearts ( groups 2 and 3 , to 49 ( 4 ) % and 50 ( 4 ) % from baseline , respectively ) and post ischaemic hearts ( group 5 , to 28 ( 8 % ) .
	manualset3
127351	1	405666	13	NULL	NULL	0	NULL	Proteasomal dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteasomal dysfunction in aging and Huntington disease .
	manualset3
127352	2	405666	13	NULL	NULL	0	NULL	Huntington disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteasomal dysfunction in aging and Huntington disease .
	manualset3
128816	3	405666	13	NULL	NULL	0	NULL	aging	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteasomal dysfunction in aging and Huntington disease .
	manualset3
127353	1	405667	13	NULL	NULL	0	NULL	Proteasome inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteasome inhibition by MG132 induces growth inhibition and death of human pulmonary fibroblast cells in a caspase-independent manner .
	manualset3
127354	2	405667	13	NULL	NULL	0	NULL	MG132	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteasome inhibition by MG132 induces growth inhibition and death of human pulmonary fibroblast cells in a caspase-independent manner .
	manualset3
127355	3	405667	13	NULL	NULL	0	NULL	growth inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteasome inhibition by MG132 induces growth inhibition and death of human pulmonary fibroblast cells in a caspase-independent manner .
	manualset3
127356	4	405667	13	NULL	NULL	0	NULL	death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteasome inhibition by MG132 induces growth inhibition and death of human pulmonary fibroblast cells in a caspase-independent manner .
	manualset3
127357	5	405667	13	NULL	NULL	0	NULL	human pulmonary fibroblast cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteasome inhibition by MG132 induces growth inhibition and death of human pulmonary fibroblast cells in a caspase-independent manner .
	manualset3
127358	6	405667	13	NULL	NULL	0	NULL	caspase-independent manner	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteasome inhibition by MG132 induces growth inhibition and death of human pulmonary fibroblast cells in a caspase-independent manner .
	manualset3
127359	1	405668	13	NULL	NULL	0	NULL	Protection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Protection is afforded to the tractor operator when a rollover protective structure ( ROPS ) is attached to the tractor .
	manualset3
127360	2	405668	13	NULL	NULL	0	NULL	tractor operator	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Protection is afforded to the tractor operator when a rollover protective structure ( ROPS ) is attached to the tractor .
	manualset3
127361	3	405668	13	NULL	NULL	0	NULL	rollover protective structure ( ROPS )	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Protection is afforded to the tractor operator when a rollover protective structure ( ROPS ) is attached to the tractor .
	manualset3
127362	4	405668	13	NULL	NULL	0	NULL	tractor 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Protection is afforded to the tractor operator when a rollover protective structure ( ROPS ) is attached to the tractor .
	manualset3
127363	1	405669	13	NULL	NULL	0	NULL	Protective cover cap	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Protective cover cap for implant attachment .
	manualset3
127364	2	405669	13	NULL	NULL	0	NULL	implant attachment	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Protective cover cap for implant attachment .
	manualset3
127365	1	405670	13	NULL	NULL	0	NULL	Protective effect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Protective effect of cyclosporin A on white matter changes in the rat brain after chronic cerebral hypoperfusion .
	manualset3
127366	2	405670	13	NULL	NULL	0	NULL	cyclosporin A	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Protective effect of cyclosporin A on white matter changes in the rat brain after chronic cerebral hypoperfusion .
	manualset3
127367	3	405670	13	NULL	NULL	0	NULL	white matter changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Protective effect of cyclosporin A on white matter changes in the rat brain after chronic cerebral hypoperfusion .
	manualset3
127368	4	405670	13	NULL	NULL	0	NULL	rat brain 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Protective effect of cyclosporin A on white matter changes in the rat brain after chronic cerebral hypoperfusion .
	manualset3
127369	5	405670	13	NULL	NULL	0	NULL	chronic cerebral hypoperfusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Protective effect of cyclosporin A on white matter changes in the rat brain after chronic cerebral hypoperfusion .
	manualset3
127370	1	405671	13	NULL	NULL	0	NULL	Protective effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Protective effect of naringin against ischemic reperfusion cerebral injury : possible neurobehavioral , biochemical and cellular alterations in rat brain .
	manualset3
127371	2	405671	13	NULL	NULL	0	NULL	naringin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Protective effect of naringin against ischemic reperfusion cerebral injury : possible neurobehavioral , biochemical and cellular alterations in rat brain .
	manualset3
127372	3	405671	13	NULL	NULL	0	NULL	ischemic reperfusion cerebral injury 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Protective effect of naringin against ischemic reperfusion cerebral injury : possible neurobehavioral , biochemical and cellular alterations in rat brain .
	manualset3
127373	4	405671	13	NULL	NULL	0	NULL	neurobehavioral alterations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Protective effect of naringin against ischemic reperfusion cerebral injury : possible neurobehavioral , biochemical and cellular alterations in rat brain .
	manualset3
127374	5	405671	13	NULL	NULL	0	NULL	biochemical alterations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Protective effect of naringin against ischemic reperfusion cerebral injury : possible neurobehavioral , biochemical and cellular alterations in rat brain .
	manualset3
127375	6	405671	13	NULL	NULL	0	NULL	cellular alterations 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Protective effect of naringin against ischemic reperfusion cerebral injury : possible neurobehavioral , biochemical and cellular alterations in rat brain .
	manualset3
127376	7	405671	13	NULL	NULL	0	NULL	rat brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Protective effect of naringin against ischemic reperfusion cerebral injury : possible neurobehavioral , biochemical and cellular alterations in rat brain .
	manualset3
127377	1	405672	13	NULL	NULL	0	NULL	Protective effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Protective effect of pentoxifylline on contrast induced nephropathy .
	manualset3
127378	2	405672	13	NULL	NULL	0	NULL	pentoxifylline	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Protective effect of pentoxifylline on contrast induced nephropathy .
	manualset3
127379	3	405672	13	NULL	NULL	0	NULL	contrast	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Protective effect of pentoxifylline on contrast induced nephropathy .
	manualset3
127380	4	405672	13	NULL	NULL	0	NULL	nephropathy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Protective effect of pentoxifylline on contrast induced nephropathy .
	manualset3
127381	1	405673	13	NULL	NULL	0	NULL	major challenge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A major challenge in evolutionary biology and plant breeding is to identify the genetic basis of complex quantitative traits , including those that contribute to adaptive variation .
	manualset3
127382	2	405673	13	NULL	NULL	0	NULL	evolutionary biology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A major challenge in evolutionary biology and plant breeding is to identify the genetic basis of complex quantitative traits , including those that contribute to adaptive variation .
	manualset3
127383	3	405673	13	NULL	NULL	0	NULL	plant	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A major challenge in evolutionary biology and plant breeding is to identify the genetic basis of complex quantitative traits , including those that contribute to adaptive variation .
	manualset3
127384	4	405673	13	NULL	NULL	0	NULL	genetic basis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A major challenge in evolutionary biology and plant breeding is to identify the genetic basis of complex quantitative traits , including those that contribute to adaptive variation .
	manualset3
127385	5	405673	13	NULL	NULL	0	NULL	complex quantitative traits	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A major challenge in evolutionary biology and plant breeding is to identify the genetic basis of complex quantitative traits , including those that contribute to adaptive variation .
	manualset3
127386	6	405673	13	NULL	NULL	0	NULL	adaptive variation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A major challenge in evolutionary biology and plant breeding is to identify the genetic basis of complex quantitative traits , including those that contribute to adaptive variation .
	manualset3
127387	1	405674	13	NULL	NULL	0	NULL	Protective eyewear	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Protective eyewear should be mandatory for athletes who are functionally 1-eyed and for athletes whose ophthalmologists recommend eye protection after eye surgery or trauma .
	manualset3
127388	2	405674	13	NULL	NULL	0	NULL	athletes 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Protective eyewear should be mandatory for athletes who are functionally 1-eyed and for athletes whose ophthalmologists recommend eye protection after eye surgery or trauma .
	manualset3
127389	3	405674	13	NULL	NULL	0	NULL	athletes 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Protective eyewear should be mandatory for athletes who are functionally 1-eyed and for athletes whose ophthalmologists recommend eye protection after eye surgery or trauma .
	manualset3
127390	4	405674	13	NULL	NULL	0	NULL	ophthalmologists 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Protective eyewear should be mandatory for athletes who are functionally 1-eyed and for athletes whose ophthalmologists recommend eye protection after eye surgery or trauma .
	manualset3
127391	5	405674	13	NULL	NULL	0	NULL	eye protection 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Protective eyewear should be mandatory for athletes who are functionally 1-eyed and for athletes whose ophthalmologists recommend eye protection after eye surgery or trauma .
	manualset3
127392	6	405674	13	NULL	NULL	0	NULL	eye surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Protective eyewear should be mandatory for athletes who are functionally 1-eyed and for athletes whose ophthalmologists recommend eye protection after eye surgery or trauma .
	manualset3
127393	7	405674	13	NULL	NULL	0	NULL	trauma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Protective eyewear should be mandatory for athletes who are functionally 1-eyed and for athletes whose ophthalmologists recommend eye protection after eye surgery or trauma .
	manualset3
127394	1	405675	13	NULL	NULL	0	NULL	Protegrin congener 64a	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Protegrin congener 64a ( PC-64a ; LTYCRRRFCVTV ) , a variant of PG-1 with 12 amino acid residues and one disulfide bond , displayed MICs of 0.45 microM ( 0.68 microg/ml ) for strain F 62 and 1.37 microM ( 2.07 microg/ml ) for strain FA 19 , which approximated those of intact PG-1 .
	manualset3
127395	2	405675	13	NULL	NULL	0	NULL	PC-64a	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Protegrin congener 64a ( PC-64a ; LTYCRRRFCVTV ) , a variant of PG-1 with 12 amino acid residues and one disulfide bond , displayed MICs of 0.45 microM ( 0.68 microg/ml ) for strain F 62 and 1.37 microM ( 2.07 microg/ml ) for strain FA 19 , which approximated those of intact PG-1 .
	manualset3
127396	3	405675	13	NULL	NULL	0	NULL	LTYCRRRFCVTV	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Protegrin congener 64a ( PC-64a ; LTYCRRRFCVTV ) , a variant of PG-1 with 12 amino acid residues and one disulfide bond , displayed MICs of 0.45 microM ( 0.68 microg/ml ) for strain F 62 and 1.37 microM ( 2.07 microg/ml ) for strain FA 19 , which approximated those of intact PG-1 .
	manualset3
127397	4	405675	13	NULL	NULL	NULL	NULL	variant of PG-1	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Protegrin congener 64a ( PC-64a ; LTYCRRRFCVTV ) , a variant of PG-1 with 12 amino acid residues and one disulfide bond , displayed MICs of 0.45 microM ( 0.68 microg/ml ) for strain F 62 and 1.37 microM ( 2.07 microg/ml ) for strain FA 19 , which approximated those of intact PG-1 .
	manualset3
127398	5	405675	13	NULL	NULL	0	NULL	12 amino acid residues 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Protegrin congener 64a ( PC-64a ; LTYCRRRFCVTV ) , a variant of PG-1 with 12 amino acid residues and one disulfide bond , displayed MICs of 0.45 microM ( 0.68 microg/ml ) for strain F 62 and 1.37 microM ( 2.07 microg/ml ) for strain FA 19 , which approximated those of intact PG-1 .
	manualset3
127399	6	405675	13	NULL	NULL	0	NULL	one disulfide bond	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Protegrin congener 64a ( PC-64a ; LTYCRRRFCVTV ) , a variant of PG-1 with 12 amino acid residues and one disulfide bond , displayed MICs of 0.45 microM ( 0.68 microg/ml ) for strain F 62 and 1.37 microM ( 2.07 microg/ml ) for strain FA 19 , which approximated those of intact PG-1 .
	manualset3
127400	7	405675	13	NULL	NULL	0	NULL	MICs	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Protegrin congener 64a ( PC-64a ; LTYCRRRFCVTV ) , a variant of PG-1 with 12 amino acid residues and one disulfide bond , displayed MICs of 0.45 microM ( 0.68 microg/ml ) for strain F 62 and 1.37 microM ( 2.07 microg/ml ) for strain FA 19 , which approximated those of intact PG-1 .
	manualset3
127401	8	405675	13	NULL	NULL	0	NULL	0.45 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Protegrin congener 64a ( PC-64a ; LTYCRRRFCVTV ) , a variant of PG-1 with 12 amino acid residues and one disulfide bond , displayed MICs of 0.45 microM ( 0.68 microg/ml ) for strain F 62 and 1.37 microM ( 2.07 microg/ml ) for strain FA 19 , which approximated those of intact PG-1 .
	manualset3
127402	9	405675	13	NULL	NULL	0	NULL	0.68 microg/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Protegrin congener 64a ( PC-64a ; LTYCRRRFCVTV ) , a variant of PG-1 with 12 amino acid residues and one disulfide bond , displayed MICs of 0.45 microM ( 0.68 microg/ml ) for strain F 62 and 1.37 microM ( 2.07 microg/ml ) for strain FA 19 , which approximated those of intact PG-1 .
	manualset3
127403	10	405675	13	NULL	NULL	0	NULL	strain F 62	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Protegrin congener 64a ( PC-64a ; LTYCRRRFCVTV ) , a variant of PG-1 with 12 amino acid residues and one disulfide bond , displayed MICs of 0.45 microM ( 0.68 microg/ml ) for strain F 62 and 1.37 microM ( 2.07 microg/ml ) for strain FA 19 , which approximated those of intact PG-1 .
	manualset3
127404	11	405675	13	NULL	NULL	0	NULL	1.37 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Protegrin congener 64a ( PC-64a ; LTYCRRRFCVTV ) , a variant of PG-1 with 12 amino acid residues and one disulfide bond , displayed MICs of 0.45 microM ( 0.68 microg/ml ) for strain F 62 and 1.37 microM ( 2.07 microg/ml ) for strain FA 19 , which approximated those of intact PG-1 .
	manualset3
127405	12	405675	13	NULL	NULL	0	NULL	2.07 microg/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Protegrin congener 64a ( PC-64a ; LTYCRRRFCVTV ) , a variant of PG-1 with 12 amino acid residues and one disulfide bond , displayed MICs of 0.45 microM ( 0.68 microg/ml ) for strain F 62 and 1.37 microM ( 2.07 microg/ml ) for strain FA 19 , which approximated those of intact PG-1 .
	manualset3
127406	13	405675	13	NULL	NULL	0	NULL	strain FA 19	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Protegrin congener 64a ( PC-64a ; LTYCRRRFCVTV ) , a variant of PG-1 with 12 amino acid residues and one disulfide bond , displayed MICs of 0.45 microM ( 0.68 microg/ml ) for strain F 62 and 1.37 microM ( 2.07 microg/ml ) for strain FA 19 , which approximated those of intact PG-1 .
	manualset3
127407	14	405675	13	NULL	NULL	NULL	NULL	PG-1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Protegrin congener 64a ( PC-64a ; LTYCRRRFCVTV ) , a variant of PG-1 with 12 amino acid residues and one disulfide bond , displayed MICs of 0.45 microM ( 0.68 microg/ml ) for strain F 62 and 1.37 microM ( 2.07 microg/ml ) for strain FA 19 , which approximated those of intact PG-1 .
	manualset3
127408	1	405676	13	NULL	NULL	0	NULL	Protein-DNA interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein-DNA interactions in this promoter were identified by dimethyl sulfate in vivo footprinting analysis of NG108-15 cells , expressing endogenous DOR .
	manualset3
127409	2	405676	13	NULL	NULL	0	NULL	promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein-DNA interactions in this promoter were identified by dimethyl sulfate in vivo footprinting analysis of NG108-15 cells , expressing endogenous DOR .
	manualset3
127410	3	405676	13	NULL	NULL	0	NULL	dimethyl sulfate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein-DNA interactions in this promoter were identified by dimethyl sulfate in vivo footprinting analysis of NG108-15 cells , expressing endogenous DOR .
	manualset3
127411	4	405676	13	NULL	NULL	0	NULL	footprinting analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein-DNA interactions in this promoter were identified by dimethyl sulfate in vivo footprinting analysis of NG108-15 cells , expressing endogenous DOR .
	manualset3
127412	5	405676	13	NULL	NULL	0	NULL	NG108-15 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein-DNA interactions in this promoter were identified by dimethyl sulfate in vivo footprinting analysis of NG108-15 cells , expressing endogenous DOR .
	manualset3
127413	6	405676	13	NULL	NULL	0	NULL	DOR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein-DNA interactions in this promoter were identified by dimethyl sulfate in vivo footprinting analysis of NG108-15 cells , expressing endogenous DOR .
	manualset3
127414	1	405677	13	NULL	NULL	0	NULL	Protein-SOH 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein-SOH are established as transient intermediates in the formation of more stable cysteine oxidation products both under basal conditions and in response to several redox-active extrinsic compounds .
	manualset3
127415	2	405677	13	NULL	NULL	0	NULL	transient intermediates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein-SOH are established as transient intermediates in the formation of more stable cysteine oxidation products both under basal conditions and in response to several redox-active extrinsic compounds .
	manualset3
127416	3	405677	13	NULL	NULL	0	NULL	formation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein-SOH are established as transient intermediates in the formation of more stable cysteine oxidation products both under basal conditions and in response to several redox-active extrinsic compounds .
	manualset3
127417	4	405677	13	NULL	NULL	0	NULL	cysteine oxidation products 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein-SOH are established as transient intermediates in the formation of more stable cysteine oxidation products both under basal conditions and in response to several redox-active extrinsic compounds .
	manualset3
127418	5	405677	13	NULL	NULL	0	NULL	basal conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein-SOH are established as transient intermediates in the formation of more stable cysteine oxidation products both under basal conditions and in response to several redox-active extrinsic compounds .
	manualset3
127419	6	405677	13	NULL	NULL	0	NULL	response	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein-SOH are established as transient intermediates in the formation of more stable cysteine oxidation products both under basal conditions and in response to several redox-active extrinsic compounds .
	manualset3
127420	7	405677	13	NULL	NULL	0	NULL	redox-active extrinsic compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein-SOH are established as transient intermediates in the formation of more stable cysteine oxidation products both under basal conditions and in response to several redox-active extrinsic compounds .
	manualset3
127421	1	405678	13	NULL	NULL	0	NULL	Protein C Yonago 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein C Yonago is a dysfunctional protein C characterized by defective anticoagulant activity determined by a coagulation assay and normal amidolytic activity measured on a synthetic substrate S-2366 ( Iijima et al. , Thromb Res 1991 ; 63 : 249 -257 ) .
	manualset3
127422	2	405678	13	NULL	NULL	0	NULL	dysfunctional protein C 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein C Yonago is a dysfunctional protein C characterized by defective anticoagulant activity determined by a coagulation assay and normal amidolytic activity measured on a synthetic substrate S-2366 ( Iijima et al. , Thromb Res 1991 ; 63 : 249 -257 ) .
	manualset3
127423	3	405678	13	NULL	NULL	0	NULL	defective anticoagulant activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein C Yonago is a dysfunctional protein C characterized by defective anticoagulant activity determined by a coagulation assay and normal amidolytic activity measured on a synthetic substrate S-2366 ( Iijima et al. , Thromb Res 1991 ; 63 : 249 -257 ) .
	manualset3
127424	4	405678	13	NULL	NULL	0	NULL	coagulation assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein C Yonago is a dysfunctional protein C characterized by defective anticoagulant activity determined by a coagulation assay and normal amidolytic activity measured on a synthetic substrate S-2366 ( Iijima et al. , Thromb Res 1991 ; 63 : 249 -257 ) .
	manualset3
127425	5	405678	13	NULL	NULL	0	NULL	amidolytic activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein C Yonago is a dysfunctional protein C characterized by defective anticoagulant activity determined by a coagulation assay and normal amidolytic activity measured on a synthetic substrate S-2366 ( Iijima et al. , Thromb Res 1991 ; 63 : 249 -257 ) .
	manualset3
127426	6	405678	13	NULL	NULL	0	NULL	synthetic substrate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein C Yonago is a dysfunctional protein C characterized by defective anticoagulant activity determined by a coagulation assay and normal amidolytic activity measured on a synthetic substrate S-2366 ( Iijima et al. , Thromb Res 1991 ; 63 : 249 -257 ) .
	manualset3
127427	7	405678	13	NULL	NULL	0	NULL	S-2366	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein C Yonago is a dysfunctional protein C characterized by defective anticoagulant activity determined by a coagulation assay and normal amidolytic activity measured on a synthetic substrate S-2366 ( Iijima et al. , Thromb Res 1991 ; 63 : 249 -257 ) .
	manualset3
127428	8	405678	13	NULL	NULL	0	NULL	Iijima 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein C Yonago is a dysfunctional protein C characterized by defective anticoagulant activity determined by a coagulation assay and normal amidolytic activity measured on a synthetic substrate S-2366 ( Iijima et al. , Thromb Res 1991 ; 63 : 249 -257 ) .
	manualset3
127429	9	405678	13	NULL	NULL	0	NULL	Thromb Res 	Journal												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein C Yonago is a dysfunctional protein C characterized by defective anticoagulant activity determined by a coagulation assay and normal amidolytic activity measured on a synthetic substrate S-2366 ( Iijima et al. , Thromb Res 1991 ; 63 : 249 -257 ) .
	manualset3
127430	10	405678	13	NULL	NULL	0	NULL	1991	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein C Yonago is a dysfunctional protein C characterized by defective anticoagulant activity determined by a coagulation assay and normal amidolytic activity measured on a synthetic substrate S-2366 ( Iijima et al. , Thromb Res 1991 ; 63 : 249 -257 ) .
	manualset3
127431	1	405679	13	NULL	NULL	0	NULL	Protein C	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein C in its activated form ( APC ) limits thrombin generation .
	manualset3
127432	2	405679	13	NULL	NULL	0	NULL	activated form ( APC )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein C in its activated form ( APC ) limits thrombin generation .
	manualset3
127434	4	405679	13	NULL	NULL	0	NULL	thrombin generation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein C in its activated form ( APC ) limits thrombin generation .
	manualset3
127435	1	405680	13	NULL	NULL	0	NULL	Protein S	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein S deficiency is a known risk factor for thrombosis .
	manualset3
127436	2	405680	13	NULL	NULL	0	NULL	deficiency 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein S deficiency is a known risk factor for thrombosis .
	manualset3
127437	3	405680	13	NULL	NULL	0	NULL	risk factor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein S deficiency is a known risk factor for thrombosis .
	manualset3
127438	4	405680	13	NULL	NULL	0	NULL	thrombosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein S deficiency is a known risk factor for thrombosis .
	manualset3
127439	1	405681	13	NULL	NULL	0	NULL	Protein biomarkers	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein biomarkers are critical for diagnosis , prognosis , and treatment of disease .
	manualset3
127440	2	405681	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein biomarkers are critical for diagnosis , prognosis , and treatment of disease .
	manualset3
127441	3	405681	13	NULL	NULL	0	NULL	prognosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein biomarkers are critical for diagnosis , prognosis , and treatment of disease .
	manualset3
127442	4	405681	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein biomarkers are critical for diagnosis , prognosis , and treatment of disease .
	manualset3
127443	5	405681	13	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein biomarkers are critical for diagnosis , prognosis , and treatment of disease .
	manualset3
127444	1	405682	13	NULL	NULL	0	NULL	Protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein concentration in EVECW and AF relative to plasma ( EV/PL and AF/PL , respectively ) was compared in the two types of edema .
	manualset3
127445	2	405682	13	NULL	NULL	0	NULL	concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein concentration in EVECW and AF relative to plasma ( EV/PL and AF/PL , respectively ) was compared in the two types of edema .
	manualset3
127446	3	405682	13	NULL	NULL	0	NULL	EVECW	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein concentration in EVECW and AF relative to plasma ( EV/PL and AF/PL , respectively ) was compared in the two types of edema .
	manualset3
127447	4	405682	13	NULL	NULL	0	NULL	AF	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein concentration in EVECW and AF relative to plasma ( EV/PL and AF/PL , respectively ) was compared in the two types of edema .
	manualset3
127448	5	405682	13	NULL	NULL	0	NULL	plasma	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein concentration in EVECW and AF relative to plasma ( EV/PL and AF/PL , respectively ) was compared in the two types of edema .
	manualset3
127449	6	405682	13	NULL	NULL	0	NULL	EV/PL	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein concentration in EVECW and AF relative to plasma ( EV/PL and AF/PL , respectively ) was compared in the two types of edema .
	manualset3
127450	7	405682	13	NULL	NULL	0	NULL	AF/PL	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein concentration in EVECW and AF relative to plasma ( EV/PL and AF/PL , respectively ) was compared in the two types of edema .
	manualset3
127451	8	405682	13	NULL	NULL	0	NULL	two types	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein concentration in EVECW and AF relative to plasma ( EV/PL and AF/PL , respectively ) was compared in the two types of edema .
	manualset3
127452	9	405682	13	NULL	NULL	0	NULL	edema	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein concentration in EVECW and AF relative to plasma ( EV/PL and AF/PL , respectively ) was compared in the two types of edema .
	manualset3
127453	1	405683	13	NULL	NULL	0	NULL	major focus	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A major focus of investigation has been the characterization of post-translational modifications ( PTMs ) of histones and the identification of the enzymes responsible .
	manualset3
127454	2	405683	13	NULL	NULL	0	NULL	investigation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A major focus of investigation has been the characterization of post-translational modifications ( PTMs ) of histones and the identification of the enzymes responsible .
	manualset3
127455	3	405683	13	NULL	NULL	0	NULL	characterization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A major focus of investigation has been the characterization of post-translational modifications ( PTMs ) of histones and the identification of the enzymes responsible .
	manualset3
127456	4	405683	13	NULL	NULL	0	NULL	post-translational modifications ( PTMs ) 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A major focus of investigation has been the characterization of post-translational modifications ( PTMs ) of histones and the identification of the enzymes responsible .
	manualset3
127457	5	405683	13	NULL	NULL	0	NULL	histones	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A major focus of investigation has been the characterization of post-translational modifications ( PTMs ) of histones and the identification of the enzymes responsible .
	manualset3
127458	6	405683	13	NULL	NULL	0	NULL	identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A major focus of investigation has been the characterization of post-translational modifications ( PTMs ) of histones and the identification of the enzymes responsible .
	manualset3
127459	7	405683	13	NULL	NULL	0	NULL	enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A major focus of investigation has been the characterization of post-translational modifications ( PTMs ) of histones and the identification of the enzymes responsible .
	manualset3
127460	1	405684	13	NULL	NULL	0	NULL	Protein denaturants	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein denaturants , urea and guanidine HCl , brought about a selective aggregation of assembly with assembly .
	manualset3
127461	2	405684	13	NULL	NULL	0	NULL	urea	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein denaturants , urea and guanidine HCl , brought about a selective aggregation of assembly with assembly .
	manualset3
127462	3	405684	13	NULL	NULL	0	NULL	guanidine HCl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein denaturants , urea and guanidine HCl , brought about a selective aggregation of assembly with assembly .
	manualset3
127463	4	405684	13	NULL	NULL	0	NULL	aggregation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein denaturants , urea and guanidine HCl , brought about a selective aggregation of assembly with assembly .
	manualset3
127464	5	405684	13	NULL	NULL	0	NULL	assembly	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein denaturants , urea and guanidine HCl , brought about a selective aggregation of assembly with assembly .
	manualset3
127465	6	405684	13	NULL	NULL	0	NULL	assembly	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein denaturants , urea and guanidine HCl , brought about a selective aggregation of assembly with assembly .
	manualset3
127466	1	405685	13	NULL	NULL	0	NULL	Protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein depletion by siRNA characterized prohibitin as an anti-apoptotic molecule in mitochondria , while the lipid binding assay demonstrated subcellular communication between mitochondria and the nucleus under oxidative stress .
	manualset3
127467	2	405685	13	NULL	NULL	0	NULL	depletion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein depletion by siRNA characterized prohibitin as an anti-apoptotic molecule in mitochondria , while the lipid binding assay demonstrated subcellular communication between mitochondria and the nucleus under oxidative stress .
	manualset3
127468	3	405685	13	NULL	NULL	0	NULL	siRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein depletion by siRNA characterized prohibitin as an anti-apoptotic molecule in mitochondria , while the lipid binding assay demonstrated subcellular communication between mitochondria and the nucleus under oxidative stress .
	manualset3
127469	4	405685	13	NULL	NULL	0	NULL	prohibitin	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein depletion by siRNA characterized prohibitin as an anti-apoptotic molecule in mitochondria , while the lipid binding assay demonstrated subcellular communication between mitochondria and the nucleus under oxidative stress .
	manualset3
127470	5	405685	13	NULL	NULL	0	NULL	anti-apoptotic molecule	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein depletion by siRNA characterized prohibitin as an anti-apoptotic molecule in mitochondria , while the lipid binding assay demonstrated subcellular communication between mitochondria and the nucleus under oxidative stress .
	manualset3
127471	6	405685	13	NULL	NULL	0	NULL	mitochondria	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein depletion by siRNA characterized prohibitin as an anti-apoptotic molecule in mitochondria , while the lipid binding assay demonstrated subcellular communication between mitochondria and the nucleus under oxidative stress .
	manualset3
127472	7	405685	13	NULL	NULL	0	NULL	lipid binding assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein depletion by siRNA characterized prohibitin as an anti-apoptotic molecule in mitochondria , while the lipid binding assay demonstrated subcellular communication between mitochondria and the nucleus under oxidative stress .
	manualset3
127473	8	405685	13	NULL	NULL	0	NULL	subcellular communication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein depletion by siRNA characterized prohibitin as an anti-apoptotic molecule in mitochondria , while the lipid binding assay demonstrated subcellular communication between mitochondria and the nucleus under oxidative stress .
	manualset3
127474	9	405685	13	NULL	NULL	0	NULL	mitochondria	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein depletion by siRNA characterized prohibitin as an anti-apoptotic molecule in mitochondria , while the lipid binding assay demonstrated subcellular communication between mitochondria and the nucleus under oxidative stress .
	manualset3
127475	10	405685	13	NULL	NULL	0	NULL	nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein depletion by siRNA characterized prohibitin as an anti-apoptotic molecule in mitochondria , while the lipid binding assay demonstrated subcellular communication between mitochondria and the nucleus under oxidative stress .
	manualset3
127476	11	405685	13	NULL	NULL	0	NULL	oxidative stress	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein depletion by siRNA characterized prohibitin as an anti-apoptotic molecule in mitochondria , while the lipid binding assay demonstrated subcellular communication between mitochondria and the nucleus under oxidative stress .
	manualset3
127477	1	405686	13	NULL	NULL	0	NULL	Protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein electrophoresis demonstrated altered electrophoretic mobility of heated bovine serum albumin .
	manualset3
127478	2	405686	13	NULL	NULL	0	NULL	electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein electrophoresis demonstrated altered electrophoretic mobility of heated bovine serum albumin .
	manualset3
127479	3	405686	13	NULL	NULL	0	NULL	electrophoretic mobility 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein electrophoresis demonstrated altered electrophoretic mobility of heated bovine serum albumin .
	manualset3
127480	4	405686	13	NULL	NULL	0	NULL	bovine serum albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein electrophoresis demonstrated altered electrophoretic mobility of heated bovine serum albumin .
	manualset3
127481	1	405687	13	NULL	NULL	0	NULL	Protein farnesyltransferase ( FTase ) inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein farnesyltransferase ( FTase ) inhibitors , generally called `` FTIs , '' block the farnesylation of prelamin A , inhibiting the biogenesis of mature lamin A and leading to an accumulation of prelamin A within cells .
	manualset3
127482	2	405687	13	NULL	NULL	0	NULL	FTIs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein farnesyltransferase ( FTase ) inhibitors , generally called `` FTIs , '' block the farnesylation of prelamin A , inhibiting the biogenesis of mature lamin A and leading to an accumulation of prelamin A within cells .
	manualset3
127484	4	405687	13	NULL	NULL	0	NULL	farnesylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein farnesyltransferase ( FTase ) inhibitors , generally called `` FTIs , '' block the farnesylation of prelamin A , inhibiting the biogenesis of mature lamin A and leading to an accumulation of prelamin A within cells .
	manualset3
127485	5	405687	13	NULL	NULL	0	NULL	prelamin A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein farnesyltransferase ( FTase ) inhibitors , generally called `` FTIs , '' block the farnesylation of prelamin A , inhibiting the biogenesis of mature lamin A and leading to an accumulation of prelamin A within cells .
	manualset3
127486	6	405687	13	NULL	NULL	0	NULL	biogenesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein farnesyltransferase ( FTase ) inhibitors , generally called `` FTIs , '' block the farnesylation of prelamin A , inhibiting the biogenesis of mature lamin A and leading to an accumulation of prelamin A within cells .
	manualset3
127487	7	405687	13	NULL	NULL	0	NULL	mature lamin A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein farnesyltransferase ( FTase ) inhibitors , generally called `` FTIs , '' block the farnesylation of prelamin A , inhibiting the biogenesis of mature lamin A and leading to an accumulation of prelamin A within cells .
	manualset3
127488	8	405687	13	NULL	NULL	0	NULL	accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein farnesyltransferase ( FTase ) inhibitors , generally called `` FTIs , '' block the farnesylation of prelamin A , inhibiting the biogenesis of mature lamin A and leading to an accumulation of prelamin A within cells .
	manualset3
127489	9	405687	13	NULL	NULL	0	NULL	prelamin A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein farnesyltransferase ( FTase ) inhibitors , generally called `` FTIs , '' block the farnesylation of prelamin A , inhibiting the biogenesis of mature lamin A and leading to an accumulation of prelamin A within cells .
	manualset3
127490	10	405687	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein farnesyltransferase ( FTase ) inhibitors , generally called `` FTIs , '' block the farnesylation of prelamin A , inhibiting the biogenesis of mature lamin A and leading to an accumulation of prelamin A within cells .
	manualset3
127491	1	405688	13	NULL	NULL	0	NULL	Protein kinase C-independent stimulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein kinase C-independent stimulation of activator protein-1 and c-Jun N-terminal kinase activity in human endometrial cancer cells by the LHRH agonist triptorelin .
	manualset3
127492	2	405688	13	NULL	NULL	0	NULL	activator protein-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein kinase C-independent stimulation of activator protein-1 and c-Jun N-terminal kinase activity in human endometrial cancer cells by the LHRH agonist triptorelin .
	manualset3
127493	3	405688	13	NULL	NULL	0	NULL	c-Jun N-terminal kinase activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein kinase C-independent stimulation of activator protein-1 and c-Jun N-terminal kinase activity in human endometrial cancer cells by the LHRH agonist triptorelin .
	manualset3
127494	4	405688	13	NULL	NULL	0	NULL	human endometrial cancer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein kinase C-independent stimulation of activator protein-1 and c-Jun N-terminal kinase activity in human endometrial cancer cells by the LHRH agonist triptorelin .
	manualset3
127495	5	405688	13	NULL	NULL	0	NULL	LHRH agonist	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein kinase C-independent stimulation of activator protein-1 and c-Jun N-terminal kinase activity in human endometrial cancer cells by the LHRH agonist triptorelin .
	manualset3
127496	6	405688	13	NULL	NULL	0	NULL	triptorelin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein kinase C-independent stimulation of activator protein-1 and c-Jun N-terminal kinase activity in human endometrial cancer cells by the LHRH agonist triptorelin .
	manualset3
127497	1	405689	13	NULL	NULL	0	NULL	Protein serine/threonine kinase sequences	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein serine/threonine kinase sequences were analyzed using Fourier transform of the coded sequences .
	manualset3
127498	2	405689	13	NULL	NULL	0	NULL	Fourier transform	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein serine/threonine kinase sequences were analyzed using Fourier transform of the coded sequences .
	manualset3
127499	3	405689	13	NULL	NULL	0	NULL	coded sequences 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein serine/threonine kinase sequences were analyzed using Fourier transform of the coded sequences .
	manualset3
127500	1	405690	13	NULL	NULL	0	NULL	Protein topology 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein topology can be described by an adjacency matrix giving information , which GSSE 's are close in space to each other and defining a graph , where GSSE 's are equivalent to vertices and interactions between them to edges .
	manualset3
127501	2	405690	13	NULL	NULL	0	NULL	adjacency matrix	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein topology can be described by an adjacency matrix giving information , which GSSE 's are close in space to each other and defining a graph , where GSSE 's are equivalent to vertices and interactions between them to edges .
	manualset3
127502	3	405690	13	NULL	NULL	0	NULL	information	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein topology can be described by an adjacency matrix giving information , which GSSE 's are close in space to each other and defining a graph , where GSSE 's are equivalent to vertices and interactions between them to edges .
	manualset3
127503	4	405690	13	NULL	NULL	0	NULL	GSSE 's 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein topology can be described by an adjacency matrix giving information , which GSSE 's are close in space to each other and defining a graph , where GSSE 's are equivalent to vertices and interactions between them to edges .
	manualset3
127504	5	405690	13	NULL	NULL	0	NULL	space	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein topology can be described by an adjacency matrix giving information , which GSSE 's are close in space to each other and defining a graph , where GSSE 's are equivalent to vertices and interactions between them to edges .
	manualset3
127505	6	405690	13	NULL	NULL	0	NULL	graph	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein topology can be described by an adjacency matrix giving information , which GSSE 's are close in space to each other and defining a graph , where GSSE 's are equivalent to vertices and interactions between them to edges .
	manualset3
127506	7	405690	13	NULL	NULL	0	NULL	GSSE 's	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein topology can be described by an adjacency matrix giving information , which GSSE 's are close in space to each other and defining a graph , where GSSE 's are equivalent to vertices and interactions between them to edges .
	manualset3
127507	8	405690	13	NULL	NULL	0	NULL	vertices	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein topology can be described by an adjacency matrix giving information , which GSSE 's are close in space to each other and defining a graph , where GSSE 's are equivalent to vertices and interactions between them to edges .
	manualset3
127508	9	405690	13	NULL	NULL	0	NULL	interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein topology can be described by an adjacency matrix giving information , which GSSE 's are close in space to each other and defining a graph , where GSSE 's are equivalent to vertices and interactions between them to edges .
	manualset3
127509	10	405690	13	NULL	NULL	0	NULL	edges	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein topology can be described by an adjacency matrix giving information , which GSSE 's are close in space to each other and defining a graph , where GSSE 's are equivalent to vertices and interactions between them to edges .
	manualset3
127510	1	405691	13	NULL	NULL	0	NULL	Proteinase inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteinase inhibitors from a mimosoideae legume , Albizzia julibrissin .
	manualset3
127511	2	405691	13	NULL	NULL	0	NULL	mimosoideae legume	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteinase inhibitors from a mimosoideae legume , Albizzia julibrissin .
	manualset3
127512	3	405691	13	NULL	NULL	0	NULL	Albizzia julibrissin	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteinase inhibitors from a mimosoideae legume , Albizzia julibrissin .
	manualset3
127513	1	405692	13	NULL	NULL	0	NULL	Proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteins are specifically recognized and ubiquitinated by the ubiquitin ligases ( E3s ) and are then degraded by the proteasome .
	manualset3
127514	2	405692	13	NULL	NULL	0	NULL	ubiquitin ligases ( E3s ) 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteins are specifically recognized and ubiquitinated by the ubiquitin ligases ( E3s ) and are then degraded by the proteasome .
	manualset3
127515	3	405692	13	NULL	NULL	0	NULL	proteasome	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteins are specifically recognized and ubiquitinated by the ubiquitin ligases ( E3s ) and are then degraded by the proteasome .
	manualset3
127516	1	405693	13	NULL	NULL	0	NULL	Proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteins of known structures are usually classified into four structural classes : all-alpha , all-beta , alpha + beta , and alpha/beta type of proteins .
	manualset3
127517	2	405693	13	NULL	NULL	0	NULL	structures	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteins of known structures are usually classified into four structural classes : all-alpha , all-beta , alpha + beta , and alpha/beta type of proteins .
	manualset3
127518	3	405693	13	NULL	NULL	0	NULL	four structural classes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteins of known structures are usually classified into four structural classes : all-alpha , all-beta , alpha + beta , and alpha/beta type of proteins .
	manualset3
127519	4	405693	13	NULL	NULL	0	NULL	all-alpha type of proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteins of known structures are usually classified into four structural classes : all-alpha , all-beta , alpha + beta , and alpha/beta type of proteins .
	manualset3
127520	5	405693	13	NULL	NULL	0	NULL	all-beta type of proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteins of known structures are usually classified into four structural classes : all-alpha , all-beta , alpha + beta , and alpha/beta type of proteins .
	manualset3
127521	6	405693	13	NULL	NULL	0	NULL	alpha + beta type of proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteins of known structures are usually classified into four structural classes : all-alpha , all-beta , alpha + beta , and alpha/beta type of proteins .
	manualset3
127522	7	405693	13	NULL	NULL	0	NULL	alpha/beta type of proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteins of known structures are usually classified into four structural classes : all-alpha , all-beta , alpha + beta , and alpha/beta type of proteins .
	manualset3
127523	1	405694	13	NULL	NULL	0	NULL	Proteomics analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteomics analysis has been used to identify markers from clinical samples from HCC patients .
	manualset3
127524	2	405694	13	NULL	NULL	0	NULL	markers 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteomics analysis has been used to identify markers from clinical samples from HCC patients .
	manualset3
127525	3	405694	13	NULL	NULL	0	NULL	clinical samples 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteomics analysis has been used to identify markers from clinical samples from HCC patients .
	manualset3
127526	4	405694	13	NULL	NULL	0	NULL	HCC patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteomics analysis has been used to identify markers from clinical samples from HCC patients .
	manualset3
127527	1	405695	13	NULL	NULL	0	NULL	Prothrombin activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Prothrombin activity was very low when measured by biological assay using physiological activators ( 7 % by one-stage method and 20 % by two-stage method ) or a Russel 's viper venom-cephalin mixture ( 23 % ) , Notechis scutatus scutatus venom ( 15 % ) and Echis carinatus venom ( 17 % ) ; in contrast , the level was found to be borderline to normal using Taipan viper venom ( 64 % ) and normal by both staphylocoagulase and immunologic methods .
	manualset3
127528	2	405695	13	NULL	NULL	0	NULL	biological assay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Prothrombin activity was very low when measured by biological assay using physiological activators ( 7 % by one-stage method and 20 % by two-stage method ) or a Russel 's viper venom-cephalin mixture ( 23 % ) , Notechis scutatus scutatus venom ( 15 % ) and Echis carinatus venom ( 17 % ) ; in contrast , the level was found to be borderline to normal using Taipan viper venom ( 64 % ) and normal by both staphylocoagulase and immunologic methods .
	manualset3
127529	3	405695	13	NULL	NULL	0	NULL	physiological activators	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Prothrombin activity was very low when measured by biological assay using physiological activators ( 7 % by one-stage method and 20 % by two-stage method ) or a Russel 's viper venom-cephalin mixture ( 23 % ) , Notechis scutatus scutatus venom ( 15 % ) and Echis carinatus venom ( 17 % ) ; in contrast , the level was found to be borderline to normal using Taipan viper venom ( 64 % ) and normal by both staphylocoagulase and immunologic methods .
	manualset3
127530	4	405695	13	NULL	NULL	0	NULL	7 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Prothrombin activity was very low when measured by biological assay using physiological activators ( 7 % by one-stage method and 20 % by two-stage method ) or a Russel 's viper venom-cephalin mixture ( 23 % ) , Notechis scutatus scutatus venom ( 15 % ) and Echis carinatus venom ( 17 % ) ; in contrast , the level was found to be borderline to normal using Taipan viper venom ( 64 % ) and normal by both staphylocoagulase and immunologic methods .
	manualset3
127531	5	405695	13	NULL	NULL	0	NULL	one-stage method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Prothrombin activity was very low when measured by biological assay using physiological activators ( 7 % by one-stage method and 20 % by two-stage method ) or a Russel 's viper venom-cephalin mixture ( 23 % ) , Notechis scutatus scutatus venom ( 15 % ) and Echis carinatus venom ( 17 % ) ; in contrast , the level was found to be borderline to normal using Taipan viper venom ( 64 % ) and normal by both staphylocoagulase and immunologic methods .
	manualset3
127532	6	405695	13	NULL	NULL	0	NULL	20 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Prothrombin activity was very low when measured by biological assay using physiological activators ( 7 % by one-stage method and 20 % by two-stage method ) or a Russel 's viper venom-cephalin mixture ( 23 % ) , Notechis scutatus scutatus venom ( 15 % ) and Echis carinatus venom ( 17 % ) ; in contrast , the level was found to be borderline to normal using Taipan viper venom ( 64 % ) and normal by both staphylocoagulase and immunologic methods .
	manualset3
127533	7	405695	13	NULL	NULL	0	NULL	two-stage method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Prothrombin activity was very low when measured by biological assay using physiological activators ( 7 % by one-stage method and 20 % by two-stage method ) or a Russel 's viper venom-cephalin mixture ( 23 % ) , Notechis scutatus scutatus venom ( 15 % ) and Echis carinatus venom ( 17 % ) ; in contrast , the level was found to be borderline to normal using Taipan viper venom ( 64 % ) and normal by both staphylocoagulase and immunologic methods .
	manualset3
127535	9	405695	13	NULL	NULL	NULL	NULL	Russel 's viper venom-cephalin mixture	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Prothrombin activity was very low when measured by biological assay using physiological activators ( 7 % by one-stage method and 20 % by two-stage method ) or a Russel 's viper venom-cephalin mixture ( 23 % ) , Notechis scutatus scutatus venom ( 15 % ) and Echis carinatus venom ( 17 % ) ; in contrast , the level was found to be borderline to normal using Taipan viper venom ( 64 % ) and normal by both staphylocoagulase and immunologic methods .
	manualset3
127536	10	405695	13	NULL	NULL	0	NULL	23 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Prothrombin activity was very low when measured by biological assay using physiological activators ( 7 % by one-stage method and 20 % by two-stage method ) or a Russel 's viper venom-cephalin mixture ( 23 % ) , Notechis scutatus scutatus venom ( 15 % ) and Echis carinatus venom ( 17 % ) ; in contrast , the level was found to be borderline to normal using Taipan viper venom ( 64 % ) and normal by both staphylocoagulase and immunologic methods .
	manualset3
127537	11	405695	13	NULL	NULL	0	NULL	Notechis scutatus scutatus venom	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Prothrombin activity was very low when measured by biological assay using physiological activators ( 7 % by one-stage method and 20 % by two-stage method ) or a Russel 's viper venom-cephalin mixture ( 23 % ) , Notechis scutatus scutatus venom ( 15 % ) and Echis carinatus venom ( 17 % ) ; in contrast , the level was found to be borderline to normal using Taipan viper venom ( 64 % ) and normal by both staphylocoagulase and immunologic methods .
	manualset3
127538	12	405695	13	NULL	NULL	0	NULL	15 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Prothrombin activity was very low when measured by biological assay using physiological activators ( 7 % by one-stage method and 20 % by two-stage method ) or a Russel 's viper venom-cephalin mixture ( 23 % ) , Notechis scutatus scutatus venom ( 15 % ) and Echis carinatus venom ( 17 % ) ; in contrast , the level was found to be borderline to normal using Taipan viper venom ( 64 % ) and normal by both staphylocoagulase and immunologic methods .
	manualset3
127539	13	405695	13	NULL	NULL	0	NULL	Echis carinatus venom 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Prothrombin activity was very low when measured by biological assay using physiological activators ( 7 % by one-stage method and 20 % by two-stage method ) or a Russel 's viper venom-cephalin mixture ( 23 % ) , Notechis scutatus scutatus venom ( 15 % ) and Echis carinatus venom ( 17 % ) ; in contrast , the level was found to be borderline to normal using Taipan viper venom ( 64 % ) and normal by both staphylocoagulase and immunologic methods .
	manualset3
127540	14	405695	13	NULL	NULL	0	NULL	17 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Prothrombin activity was very low when measured by biological assay using physiological activators ( 7 % by one-stage method and 20 % by two-stage method ) or a Russel 's viper venom-cephalin mixture ( 23 % ) , Notechis scutatus scutatus venom ( 15 % ) and Echis carinatus venom ( 17 % ) ; in contrast , the level was found to be borderline to normal using Taipan viper venom ( 64 % ) and normal by both staphylocoagulase and immunologic methods .
	manualset3
127541	15	405695	13	NULL	NULL	0	NULL	contrast	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Prothrombin activity was very low when measured by biological assay using physiological activators ( 7 % by one-stage method and 20 % by two-stage method ) or a Russel 's viper venom-cephalin mixture ( 23 % ) , Notechis scutatus scutatus venom ( 15 % ) and Echis carinatus venom ( 17 % ) ; in contrast , the level was found to be borderline to normal using Taipan viper venom ( 64 % ) and normal by both staphylocoagulase and immunologic methods .
	manualset3
127542	16	405695	13	NULL	NULL	0	NULL	level	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Prothrombin activity was very low when measured by biological assay using physiological activators ( 7 % by one-stage method and 20 % by two-stage method ) or a Russel 's viper venom-cephalin mixture ( 23 % ) , Notechis scutatus scutatus venom ( 15 % ) and Echis carinatus venom ( 17 % ) ; in contrast , the level was found to be borderline to normal using Taipan viper venom ( 64 % ) and normal by both staphylocoagulase and immunologic methods .
	manualset3
127543	17	405695	13	NULL	NULL	0	NULL	Taipan viper venom	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Prothrombin activity was very low when measured by biological assay using physiological activators ( 7 % by one-stage method and 20 % by two-stage method ) or a Russel 's viper venom-cephalin mixture ( 23 % ) , Notechis scutatus scutatus venom ( 15 % ) and Echis carinatus venom ( 17 % ) ; in contrast , the level was found to be borderline to normal using Taipan viper venom ( 64 % ) and normal by both staphylocoagulase and immunologic methods .
	manualset3
127544	18	405695	13	NULL	NULL	0	NULL	64 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Prothrombin activity was very low when measured by biological assay using physiological activators ( 7 % by one-stage method and 20 % by two-stage method ) or a Russel 's viper venom-cephalin mixture ( 23 % ) , Notechis scutatus scutatus venom ( 15 % ) and Echis carinatus venom ( 17 % ) ; in contrast , the level was found to be borderline to normal using Taipan viper venom ( 64 % ) and normal by both staphylocoagulase and immunologic methods .
	manualset3
127545	19	405695	13	NULL	NULL	0	NULL	staphylocoagulase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Prothrombin activity was very low when measured by biological assay using physiological activators ( 7 % by one-stage method and 20 % by two-stage method ) or a Russel 's viper venom-cephalin mixture ( 23 % ) , Notechis scutatus scutatus venom ( 15 % ) and Echis carinatus venom ( 17 % ) ; in contrast , the level was found to be borderline to normal using Taipan viper venom ( 64 % ) and normal by both staphylocoagulase and immunologic methods .
	manualset3
127546	20	405695	13	NULL	NULL	0	NULL	immunologic methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Prothrombin activity was very low when measured by biological assay using physiological activators ( 7 % by one-stage method and 20 % by two-stage method ) or a Russel 's viper venom-cephalin mixture ( 23 % ) , Notechis scutatus scutatus venom ( 15 % ) and Echis carinatus venom ( 17 % ) ; in contrast , the level was found to be borderline to normal using Taipan viper venom ( 64 % ) and normal by both staphylocoagulase and immunologic methods .
	manualset3
127547	1	405696	13	NULL	NULL	0	NULL	Proto-oncogene c-ros	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Proto-oncogene c-ros codes for a receptor-type protein tyrosine kinase ( PTK ) sharing high homology with the Drosophila sevenless protein .
	manualset3
127549	3	405696	13	NULL	NULL	0	NULL	 receptor-type protein tyrosine kinase ( PTK )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Proto-oncogene c-ros codes for a receptor-type protein tyrosine kinase ( PTK ) sharing high homology with the Drosophila sevenless protein .
	manualset3
127550	4	405696	13	NULL	NULL	0	NULL	homology	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Proto-oncogene c-ros codes for a receptor-type protein tyrosine kinase ( PTK ) sharing high homology with the Drosophila sevenless protein .
	manualset3
127551	5	405696	13	NULL	NULL	0	NULL	Drosophila sevenless protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Proto-oncogene c-ros codes for a receptor-type protein tyrosine kinase ( PTK ) sharing high homology with the Drosophila sevenless protein .
	manualset3
127552	1	405697	13	NULL	NULL	0	NULL	Protocol	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Protocol availability and use did not affect patient outcomes .
	manualset3
127553	2	405697	13	NULL	NULL	0	NULL	availability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Protocol availability and use did not affect patient outcomes .
	manualset3
127554	3	405697	13	NULL	NULL	0	NULL	use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Protocol availability and use did not affect patient outcomes .
	manualset3
127555	4	405697	13	NULL	NULL	0	NULL	patient outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Protocol availability and use did not affect patient outcomes .
	manualset3
127556	1	405698	13	NULL	NULL	0	NULL	Proton MR spectra	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton MR spectra were obtained from a trunk phantom and 23 volunteers using a single free induction decay measurement .
	manualset3
127557	2	405698	13	NULL	NULL	0	NULL	 trunk phantom	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton MR spectra were obtained from a trunk phantom and 23 volunteers using a single free induction decay measurement .
	manualset3
127558	3	405698	13	NULL	NULL	0	NULL	23 volunteers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton MR spectra were obtained from a trunk phantom and 23 volunteers using a single free induction decay measurement .
	manualset3
127559	4	405698	13	NULL	NULL	0	NULL	induction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton MR spectra were obtained from a trunk phantom and 23 volunteers using a single free induction decay measurement .
	manualset3
127560	5	405698	13	NULL	NULL	0	NULL	decay measurement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton MR spectra were obtained from a trunk phantom and 23 volunteers using a single free induction decay measurement .
	manualset3
127561	1	405699	13	NULL	NULL	0	NULL	Proton magnetic resonance spectroscopy ( ( 1 ) H-MRS )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton magnetic resonance spectroscopy ( ( 1 ) H-MRS ) is a noninvasive technique that can quantify biochemical compounds in the brain .
	manualset3
127562	2	405699	13	NULL	NULL	0	NULL	technique 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton magnetic resonance spectroscopy ( ( 1 ) H-MRS ) is a noninvasive technique that can quantify biochemical compounds in the brain .
	manualset3
127563	3	405699	13	NULL	NULL	0	NULL	biochemical compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton magnetic resonance spectroscopy ( ( 1 ) H-MRS ) is a noninvasive technique that can quantify biochemical compounds in the brain .
	manualset3
127564	4	405699	13	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton magnetic resonance spectroscopy ( ( 1 ) H-MRS ) is a noninvasive technique that can quantify biochemical compounds in the brain .
	manualset3
127565	1	405700	13	NULL	NULL	0	NULL	Proton permeability coefficients	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton and calcium permeability coefficients of large unilamellar vesicles made from natural complex mixtures of phospholipids were measured in various conditions and related to membrane fluidity .
	manualset3
127566	2	405700	13	NULL	NULL	0	NULL	calcium permeability coefficients	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton and calcium permeability coefficients of large unilamellar vesicles made from natural complex mixtures of phospholipids were measured in various conditions and related to membrane fluidity .
	manualset3
127567	3	405700	13	NULL	NULL	0	NULL	large unilamellar vesicles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton and calcium permeability coefficients of large unilamellar vesicles made from natural complex mixtures of phospholipids were measured in various conditions and related to membrane fluidity .
	manualset3
127568	4	405700	13	NULL	NULL	0	NULL	natural complex mixtures 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton and calcium permeability coefficients of large unilamellar vesicles made from natural complex mixtures of phospholipids were measured in various conditions and related to membrane fluidity .
	manualset3
127569	5	405700	13	NULL	NULL	0	NULL	phospholipids 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton and calcium permeability coefficients of large unilamellar vesicles made from natural complex mixtures of phospholipids were measured in various conditions and related to membrane fluidity .
	manualset3
127570	6	405700	13	NULL	NULL	0	NULL	various conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton and calcium permeability coefficients of large unilamellar vesicles made from natural complex mixtures of phospholipids were measured in various conditions and related to membrane fluidity .
	manualset3
127571	7	405700	13	NULL	NULL	0	NULL	membrane fluidity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton and calcium permeability coefficients of large unilamellar vesicles made from natural complex mixtures of phospholipids were measured in various conditions and related to membrane fluidity .
	manualset3
127572	1	405701	13	NULL	NULL	0	NULL	Protons	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Protons and how they are transported by proton pumps .
	manualset3
127573	2	405701	13	NULL	NULL	0	NULL	proton pumps	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Protons and how they are transported by proton pumps .
	manualset3
127574	1	405702	13	NULL	NULL	0	NULL	Protozoa	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Protozoa were labeled by incubating 100 ml rumen fluid with ( 14C ) choline for 1 h. The protozoa were concentrated by centrifugation and then washed with rumen fluid .
	manualset3
127575	2	405702	13	NULL	NULL	0	NULL	100 ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Protozoa were labeled by incubating 100 ml rumen fluid with ( 14C ) choline for 1 h. The protozoa were concentrated by centrifugation and then washed with rumen fluid .
	manualset3
127576	3	405702	13	NULL	NULL	0	NULL	rumen fluid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Protozoa were labeled by incubating 100 ml rumen fluid with ( 14C ) choline for 1 h. The protozoa were concentrated by centrifugation and then washed with rumen fluid .
	manualset3
127577	4	405702	13	NULL	NULL	0	NULL	14C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Protozoa were labeled by incubating 100 ml rumen fluid with ( 14C ) choline for 1 h. The protozoa were concentrated by centrifugation and then washed with rumen fluid .
	manualset3
127578	5	405702	13	NULL	NULL	0	NULL	choline 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Protozoa were labeled by incubating 100 ml rumen fluid with ( 14C ) choline for 1 h. The protozoa were concentrated by centrifugation and then washed with rumen fluid .
	manualset3
127579	6	405702	13	NULL	NULL	0	NULL	1 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Protozoa were labeled by incubating 100 ml rumen fluid with ( 14C ) choline for 1 h. The protozoa were concentrated by centrifugation and then washed with rumen fluid .
	manualset3
127580	7	405702	13	NULL	NULL	0	NULL	protozoa	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Protozoa were labeled by incubating 100 ml rumen fluid with ( 14C ) choline for 1 h. The protozoa were concentrated by centrifugation and then washed with rumen fluid .
	manualset3
127581	8	405702	13	NULL	NULL	0	NULL	centrifugation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Protozoa were labeled by incubating 100 ml rumen fluid with ( 14C ) choline for 1 h. The protozoa were concentrated by centrifugation and then washed with rumen fluid .
	manualset3
127582	9	405702	13	NULL	NULL	0	NULL	rumen fluid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Protozoa were labeled by incubating 100 ml rumen fluid with ( 14C ) choline for 1 h. The protozoa were concentrated by centrifugation and then washed with rumen fluid .
	manualset3
127583	1	405703	13	NULL	NULL	0	NULL	major role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A major role in the diagnosis of sarcoidosis is played by histologic evidence on the basis of which additional tests can be used .
	manualset3
127584	2	405703	13	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A major role in the diagnosis of sarcoidosis is played by histologic evidence on the basis of which additional tests can be used .
	manualset3
127585	3	405703	13	NULL	NULL	0	NULL	sarcoidosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A major role in the diagnosis of sarcoidosis is played by histologic evidence on the basis of which additional tests can be used .
	manualset3
127586	4	405703	13	NULL	NULL	0	NULL	histologic evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A major role in the diagnosis of sarcoidosis is played by histologic evidence on the basis of which additional tests can be used .
	manualset3
127587	5	405703	13	NULL	NULL	0	NULL	basis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A major role in the diagnosis of sarcoidosis is played by histologic evidence on the basis of which additional tests can be used .
	manualset3
127588	6	405703	13	NULL	NULL	0	NULL	additional tests 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A major role in the diagnosis of sarcoidosis is played by histologic evidence on the basis of which additional tests can be used .
	manualset3
127589	1	405704	13	NULL	NULL	0	NULL	patient care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Providing patient care based on the best evidence is a priority for healthcare institutions across the country to improve practice and patient outcomes .
	manualset3
127590	2	405704	13	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Providing patient care based on the best evidence is a priority for healthcare institutions across the country to improve practice and patient outcomes .
	manualset3
127591	3	405704	13	NULL	NULL	0	NULL	priority	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Providing patient care based on the best evidence is a priority for healthcare institutions across the country to improve practice and patient outcomes .
	manualset3
127592	4	405704	13	NULL	NULL	0	NULL	healthcare institutions	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Providing patient care based on the best evidence is a priority for healthcare institutions across the country to improve practice and patient outcomes .
	manualset3
127593	5	405704	13	NULL	NULL	0	NULL	country 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Providing patient care based on the best evidence is a priority for healthcare institutions across the country to improve practice and patient outcomes .
	manualset3
127594	6	405704	13	NULL	NULL	0	NULL	practice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Providing patient care based on the best evidence is a priority for healthcare institutions across the country to improve practice and patient outcomes .
	manualset3
127595	7	405704	13	NULL	NULL	0	NULL	patient outcomes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Providing patient care based on the best evidence is a priority for healthcare institutions across the country to improve practice and patient outcomes .
	manualset3
127596	1	405705	13	NULL	NULL	0	NULL	Provision	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Provision of appropriate staff training may be a key to expanding EoL program participation in skilled nursing .
	manualset3
127597	2	405705	13	NULL	NULL	0	NULL	staff 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Provision of appropriate staff training may be a key to expanding EoL program participation in skilled nursing .
	manualset3
127598	3	405705	13	NULL	NULL	0	NULL	training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Provision of appropriate staff training may be a key to expanding EoL program participation in skilled nursing .
	manualset3
127599	4	405705	13	NULL	NULL	0	NULL	EoL program	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Provision of appropriate staff training may be a key to expanding EoL program participation in skilled nursing .
	manualset3
127600	5	405705	13	NULL	NULL	0	NULL	participation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Provision of appropriate staff training may be a key to expanding EoL program participation in skilled nursing .
	manualset3
128817	6	405705	13	NULL	NULL	0	NULL	skilled nursing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Provision of appropriate staff training may be a key to expanding EoL program participation in skilled nursing .
	manualset3
127601	1	405706	13	NULL	NULL	0	NULL	Provocation tests	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Provocation tests should be performed to plan avoidance measures in latex-allergic children especially before surgical interventions .
	manualset3
127602	2	405706	13	NULL	NULL	0	NULL	avoidance measures 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Provocation tests should be performed to plan avoidance measures in latex-allergic children especially before surgical interventions .
	manualset3
127603	3	405706	13	NULL	NULL	0	NULL	latex-allergic children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Provocation tests should be performed to plan avoidance measures in latex-allergic children especially before surgical interventions .
	manualset3
127604	4	405706	13	NULL	NULL	0	NULL	surgical interventions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Provocation tests should be performed to plan avoidance measures in latex-allergic children especially before surgical interventions .
	manualset3
127605	1	405707	13	NULL	NULL	0	NULL	Proximate composition	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Proximate composition and mineral content of selected Tanzanian vegetables and the effect of traditional processing on the retention of ascorbic acid , riboflavin and thiamine .
	manualset3
127606	2	405707	13	NULL	NULL	0	NULL	mineral content	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Proximate composition and mineral content of selected Tanzanian vegetables and the effect of traditional processing on the retention of ascorbic acid , riboflavin and thiamine .
	manualset3
127607	3	405707	13	NULL	NULL	0	NULL	Tanzanian vegetables	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Proximate composition and mineral content of selected Tanzanian vegetables and the effect of traditional processing on the retention of ascorbic acid , riboflavin and thiamine .
	manualset3
127608	4	405707	13	NULL	NULL	0	NULL	traditional processing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Proximate composition and mineral content of selected Tanzanian vegetables and the effect of traditional processing on the retention of ascorbic acid , riboflavin and thiamine .
	manualset3
127609	5	405707	13	NULL	NULL	0	NULL	retention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Proximate composition and mineral content of selected Tanzanian vegetables and the effect of traditional processing on the retention of ascorbic acid , riboflavin and thiamine .
	manualset3
127610	6	405707	13	NULL	NULL	0	NULL	ascorbic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Proximate composition and mineral content of selected Tanzanian vegetables and the effect of traditional processing on the retention of ascorbic acid , riboflavin and thiamine .
	manualset3
127611	7	405707	13	NULL	NULL	0	NULL	riboflavin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Proximate composition and mineral content of selected Tanzanian vegetables and the effect of traditional processing on the retention of ascorbic acid , riboflavin and thiamine .
	manualset3
127612	8	405707	13	NULL	NULL	0	NULL	thiamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Proximate composition and mineral content of selected Tanzanian vegetables and the effect of traditional processing on the retention of ascorbic acid , riboflavin and thiamine .
	manualset3
127613	1	405708	13	NULL	NULL	0	NULL	Psammaplin A ( 11c ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Psammaplin A ( 11c ) is a marine metabolite previously reported to be a potent inhibitor of two classes of epigenetic enzymes : histone deacetylases and DNA methyltransferases .
	manualset3
127614	2	405708	13	NULL	NULL	0	NULL	marine metabolite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Psammaplin A ( 11c ) is a marine metabolite previously reported to be a potent inhibitor of two classes of epigenetic enzymes : histone deacetylases and DNA methyltransferases .
	manualset3
127615	3	405708	13	NULL	NULL	0	NULL	inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Psammaplin A ( 11c ) is a marine metabolite previously reported to be a potent inhibitor of two classes of epigenetic enzymes : histone deacetylases and DNA methyltransferases .
	manualset3
127616	4	405708	13	NULL	NULL	0	NULL	two classes 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Psammaplin A ( 11c ) is a marine metabolite previously reported to be a potent inhibitor of two classes of epigenetic enzymes : histone deacetylases and DNA methyltransferases .
	manualset3
127617	5	405708	13	NULL	NULL	0	NULL	epigenetic enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Psammaplin A ( 11c ) is a marine metabolite previously reported to be a potent inhibitor of two classes of epigenetic enzymes : histone deacetylases and DNA methyltransferases .
	manualset3
127618	6	405708	13	NULL	NULL	0	NULL	histone deacetylases 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Psammaplin A ( 11c ) is a marine metabolite previously reported to be a potent inhibitor of two classes of epigenetic enzymes : histone deacetylases and DNA methyltransferases .
	manualset3
127619	7	405708	13	NULL	NULL	0	NULL	DNA methyltransferases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Psammaplin A ( 11c ) is a marine metabolite previously reported to be a potent inhibitor of two classes of epigenetic enzymes : histone deacetylases and DNA methyltransferases .
	manualset3
127620	1	405709	13	NULL	NULL	0	NULL	Pseudo-ternary phase diagrams	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Pseudo-ternary phase diagrams were constructed to evaluate the phase behavior of the w/o microemulsion .
	manualset3
127621	2	405709	13	NULL	NULL	0	NULL	phase behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pseudo-ternary phase diagrams were constructed to evaluate the phase behavior of the w/o microemulsion .
	manualset3
127622	3	405709	13	NULL	NULL	0	NULL	w/o microemulsion 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Pseudo-ternary phase diagrams were constructed to evaluate the phase behavior of the w/o microemulsion .
	manualset3
127623	1	405710	13	NULL	NULL	0	NULL	Pseudomonad swarming motility	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pseudomonad swarming motility is restricted to a narrow range of high matric water potentials .
	manualset3
127624	2	405710	13	NULL	NULL	0	NULL	narrow range	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pseudomonad swarming motility is restricted to a narrow range of high matric water potentials .
	manualset3
127625	3	405710	13	NULL	NULL	0	NULL	high matric water potentials	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pseudomonad swarming motility is restricted to a narrow range of high matric water potentials .
	manualset3
127626	1	405711	13	NULL	NULL	0	NULL	Pseudomonas aeruginosa endophthalmitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pseudomonas aeruginosa endophthalmitis after penetrating keratoplasty transmitted from the same donor to two recipients confirmed by pulsed-field gel electrophoresis .
	manualset3
127627	2	405711	13	NULL	NULL	0	NULL	penetrating keratoplasty	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pseudomonas aeruginosa endophthalmitis after penetrating keratoplasty transmitted from the same donor to two recipients confirmed by pulsed-field gel electrophoresis .
	manualset3
127628	3	405711	13	NULL	NULL	0	NULL	donor 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Pseudomonas aeruginosa endophthalmitis after penetrating keratoplasty transmitted from the same donor to two recipients confirmed by pulsed-field gel electrophoresis .
	manualset3
127629	4	405711	13	NULL	NULL	0	NULL	two recipients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Pseudomonas aeruginosa endophthalmitis after penetrating keratoplasty transmitted from the same donor to two recipients confirmed by pulsed-field gel electrophoresis .
	manualset3
127630	5	405711	13	NULL	NULL	0	NULL	pulsed-field gel electrophoresis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pseudomonas aeruginosa endophthalmitis after penetrating keratoplasty transmitted from the same donor to two recipients confirmed by pulsed-field gel electrophoresis .
	manualset3
127631	1	405712	13	NULL	NULL	0	NULL	Pseudoxanthoma elasticum ( PXE ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pseudoxanthoma elasticum ( PXE ) , a prototypic heritable disorder with ectopic mineralization , manifests with characteristic skin findings , ocular involvement , and cardiovascular problems .
	manualset3
127632	2	405712	13	NULL	NULL	0	NULL	 prototypic heritable disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pseudoxanthoma elasticum ( PXE ) , a prototypic heritable disorder with ectopic mineralization , manifests with characteristic skin findings , ocular involvement , and cardiovascular problems .
	manualset3
127633	3	405712	13	NULL	NULL	0	NULL	ectopic mineralization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pseudoxanthoma elasticum ( PXE ) , a prototypic heritable disorder with ectopic mineralization , manifests with characteristic skin findings , ocular involvement , and cardiovascular problems .
	manualset3
127635	5	405712	13	NULL	NULL	0	NULL	characteristic skin findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pseudoxanthoma elasticum ( PXE ) , a prototypic heritable disorder with ectopic mineralization , manifests with characteristic skin findings , ocular involvement , and cardiovascular problems .
	manualset3
127636	6	405712	13	NULL	NULL	0	NULL	ocular involvement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pseudoxanthoma elasticum ( PXE ) , a prototypic heritable disorder with ectopic mineralization , manifests with characteristic skin findings , ocular involvement , and cardiovascular problems .
	manualset3
127637	7	405712	13	NULL	NULL	0	NULL	cardiovascular problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pseudoxanthoma elasticum ( PXE ) , a prototypic heritable disorder with ectopic mineralization , manifests with characteristic skin findings , ocular involvement , and cardiovascular problems .
	manualset3
127638	1	405713	13	NULL	NULL	0	NULL	Psoas abscess	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Psoas abscess was the first sign of Crohn 's disease in 11 of 46 reported patients .
	manualset3
127639	2	405713	13	NULL	NULL	0	NULL	first sign	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Psoas abscess was the first sign of Crohn 's disease in 11 of 46 reported patients .
	manualset3
127640	3	405713	13	NULL	NULL	0	NULL	Crohn 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Psoas abscess was the first sign of Crohn 's disease in 11 of 46 reported patients .
	manualset3
127641	4	405713	13	NULL	NULL	0	NULL	11 of 46 reported patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Psoas abscess was the first sign of Crohn 's disease in 11 of 46 reported patients .
	manualset3
127642	1	405714	13	NULL	NULL	0	NULL	Psychiatric disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychiatric disorders during pregnancy are associated with poor obstetric outcomes , higher risk of postpartum psychiatric illness , increased rates of substance abuse , lower participation in prenatal care , and adverse infant and family outcomes .
	manualset3
127643	2	405714	13	NULL	NULL	0	NULL	pregnancy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychiatric disorders during pregnancy are associated with poor obstetric outcomes , higher risk of postpartum psychiatric illness , increased rates of substance abuse , lower participation in prenatal care , and adverse infant and family outcomes .
	manualset3
127644	3	405714	13	NULL	NULL	0	NULL	poor obstetric outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychiatric disorders during pregnancy are associated with poor obstetric outcomes , higher risk of postpartum psychiatric illness , increased rates of substance abuse , lower participation in prenatal care , and adverse infant and family outcomes .
	manualset3
127645	4	405714	13	NULL	NULL	0	NULL	higher risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychiatric disorders during pregnancy are associated with poor obstetric outcomes , higher risk of postpartum psychiatric illness , increased rates of substance abuse , lower participation in prenatal care , and adverse infant and family outcomes .
	manualset3
127646	5	405714	13	NULL	NULL	0	NULL	postpartum psychiatric illness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychiatric disorders during pregnancy are associated with poor obstetric outcomes , higher risk of postpartum psychiatric illness , increased rates of substance abuse , lower participation in prenatal care , and adverse infant and family outcomes .
	manualset3
127647	6	405714	13	NULL	NULL	0	NULL	 rates of substance abuse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychiatric disorders during pregnancy are associated with poor obstetric outcomes , higher risk of postpartum psychiatric illness , increased rates of substance abuse , lower participation in prenatal care , and adverse infant and family outcomes .
	manualset3
127648	7	405714	13	NULL	NULL	0	NULL	lower participation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychiatric disorders during pregnancy are associated with poor obstetric outcomes , higher risk of postpartum psychiatric illness , increased rates of substance abuse , lower participation in prenatal care , and adverse infant and family outcomes .
	manualset3
127649	8	405714	13	NULL	NULL	0	NULL	prenatal care 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychiatric disorders during pregnancy are associated with poor obstetric outcomes , higher risk of postpartum psychiatric illness , increased rates of substance abuse , lower participation in prenatal care , and adverse infant and family outcomes .
	manualset3
127650	9	405714	13	NULL	NULL	0	NULL	adverse infant outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychiatric disorders during pregnancy are associated with poor obstetric outcomes , higher risk of postpartum psychiatric illness , increased rates of substance abuse , lower participation in prenatal care , and adverse infant and family outcomes .
	manualset3
127651	10	405714	13	NULL	NULL	0	NULL	adverse family outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychiatric disorders during pregnancy are associated with poor obstetric outcomes , higher risk of postpartum psychiatric illness , increased rates of substance abuse , lower participation in prenatal care , and adverse infant and family outcomes .
	manualset3
127652	1	405715	13	NULL	NULL	0	NULL	Psychiatric issues	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychiatric issues in renal dialysis and transplantation .
	manualset3
127653	2	405715	13	NULL	NULL	0	NULL	renal dialysis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychiatric issues in renal dialysis and transplantation .
	manualset3
127654	3	405715	13	NULL	NULL	0	NULL	transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychiatric issues in renal dialysis and transplantation .
	manualset3
127655	1	405716	13	NULL	NULL	0	NULL	Psychiatric nurses 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychiatric nurses ' attitudes towards patient autonomy in depot clinics .
	manualset3
127656	2	405716	13	NULL	NULL	0	NULL	attitudes	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychiatric nurses ' attitudes towards patient autonomy in depot clinics .
	manualset3
127657	3	405716	13	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychiatric nurses ' attitudes towards patient autonomy in depot clinics .
	manualset3
127658	4	405716	13	NULL	NULL	0	NULL	autonomy 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychiatric nurses ' attitudes towards patient autonomy in depot clinics .
	manualset3
127659	5	405716	13	NULL	NULL	0	NULL	depot clinics	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychiatric nurses ' attitudes towards patient autonomy in depot clinics .
	manualset3
127660	1	405717	13	NULL	NULL	0	NULL	Psychodynamic psychiatry 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychodynamic psychiatry , particularly a psychodynamic orientation is uniquely helpful in complex , community-based clinical situations .
	manualset3
127661	2	405717	13	NULL	NULL	0	NULL	psychodynamic orientation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychodynamic psychiatry , particularly a psychodynamic orientation is uniquely helpful in complex , community-based clinical situations .
	manualset3
127662	3	405717	13	NULL	NULL	0	NULL	community-based clinical situations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychodynamic psychiatry , particularly a psychodynamic orientation is uniquely helpful in complex , community-based clinical situations .
	manualset3
127663	1	405718	13	NULL	NULL	0	NULL	Psychoendocrinological studies 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychoendocrinological studies have focused on the hypothalamic-pituitary-adrenal axis in patients with depression .
	manualset3
127664	2	405718	13	NULL	NULL	0	NULL	hypothalamic-pituitary-adrenal axis 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychoendocrinological studies have focused on the hypothalamic-pituitary-adrenal axis in patients with depression .
	manualset3
127665	3	405718	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychoendocrinological studies have focused on the hypothalamic-pituitary-adrenal axis in patients with depression .
	manualset3
127666	4	405718	13	NULL	NULL	0	NULL	depression 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychoendocrinological studies have focused on the hypothalamic-pituitary-adrenal axis in patients with depression .
	manualset3
127667	1	405719	13	NULL	NULL	0	NULL	Yucatan micropig 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A male uncastrated Yucatan micropig ( 27.2 kg ) was given a 1 g dose of antipyrine intravenously .
	manualset3
127668	2	405719	13	NULL	NULL	0	NULL	27.2 kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A male uncastrated Yucatan micropig ( 27.2 kg ) was given a 1 g dose of antipyrine intravenously .
	manualset3
127669	3	405719	13	NULL	NULL	0	NULL	1 g dose	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A male uncastrated Yucatan micropig ( 27.2 kg ) was given a 1 g dose of antipyrine intravenously .
	manualset3
127670	4	405719	13	NULL	NULL	0	NULL	antipyrine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A male uncastrated Yucatan micropig ( 27.2 kg ) was given a 1 g dose of antipyrine intravenously .
	manualset3
127671	1	405720	13	NULL	NULL	0	NULL	Psychogenic purpura	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychogenic purpura : a most distressing case .
	manualset3
127672	2	405720	13	NULL	NULL	0	NULL	distressing case 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychogenic purpura : a most distressing case .
	manualset3
127673	1	405721	13	NULL	NULL	0	NULL	Psychological effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychological effects of implantable cardioverter-defibrillator leads under advisory .
	manualset3
127674	2	405721	13	NULL	NULL	NULL	NULL	implantable cardioverter-defibrillator leads	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Psychological effects of implantable cardioverter-defibrillator leads under advisory .
	manualset3
127675	1	405722	13	NULL	NULL	0	NULL	Psychometric properties	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychometric properties of the twelve item World Health Organization Disability Assessment Schedule II ( WHO-DAS II ) in Spanish primary care patients with a first major depressive episode .
	manualset3
127677	3	405722	13	NULL	NULL	NULL	NULL	twelve item World Health Organization Disability Assessment Schedule II ( WHO-DAS II )	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Psychometric properties of the twelve item World Health Organization Disability Assessment Schedule II ( WHO-DAS II ) in Spanish primary care patients with a first major depressive episode .
	manualset3
127678	4	405722	13	NULL	NULL	0	NULL	Spanish primary care patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychometric properties of the twelve item World Health Organization Disability Assessment Schedule II ( WHO-DAS II ) in Spanish primary care patients with a first major depressive episode .
	manualset3
127679	5	405722	13	NULL	NULL	0	NULL	depressive episode	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychometric properties of the twelve item World Health Organization Disability Assessment Schedule II ( WHO-DAS II ) in Spanish primary care patients with a first major depressive episode .
	manualset3
127680	1	405723	13	NULL	NULL	0	NULL	Psychopharmacologic management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychopharmacologic management during cancer treatment .
	manualset3
127681	2	405723	13	NULL	NULL	0	NULL	cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychopharmacologic management during cancer treatment .
	manualset3
127682	3	405723	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychopharmacologic management during cancer treatment .
	manualset3
127683	1	405724	13	NULL	NULL	0	NULL	mammalian expression vector	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A mammalian expression vector containing the bacterial chloramphenicol acetyltransferase ( CAT ) gene was used to demonstrate that CAT could be successfully used as a reporter system in fish cells growing at low temperatures .
	manualset3
127684	2	405724	13	NULL	NULL	0	NULL	bacterial chloramphenicol acetyltransferase ( CAT ) gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A mammalian expression vector containing the bacterial chloramphenicol acetyltransferase ( CAT ) gene was used to demonstrate that CAT could be successfully used as a reporter system in fish cells growing at low temperatures .
	manualset3
127685	3	405724	13	NULL	NULL	0	NULL	CAT	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A mammalian expression vector containing the bacterial chloramphenicol acetyltransferase ( CAT ) gene was used to demonstrate that CAT could be successfully used as a reporter system in fish cells growing at low temperatures .
	manualset3
127686	4	405724	13	NULL	NULL	0	NULL	reporter system 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A mammalian expression vector containing the bacterial chloramphenicol acetyltransferase ( CAT ) gene was used to demonstrate that CAT could be successfully used as a reporter system in fish cells growing at low temperatures .
	manualset3
127687	5	405724	13	NULL	NULL	0	NULL	fish cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A mammalian expression vector containing the bacterial chloramphenicol acetyltransferase ( CAT ) gene was used to demonstrate that CAT could be successfully used as a reporter system in fish cells growing at low temperatures .
	manualset3
127688	6	405724	13	NULL	NULL	0	NULL	temperatures 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A mammalian expression vector containing the bacterial chloramphenicol acetyltransferase ( CAT ) gene was used to demonstrate that CAT could be successfully used as a reporter system in fish cells growing at low temperatures .
	manualset3
127689	1	405725	13	NULL	NULL	0	NULL	Psychosocial risk factors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychosocial risk factors for obesity among women in a family planning clinic .
	manualset3
127690	2	405725	13	NULL	NULL	0	NULL	obesity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychosocial risk factors for obesity among women in a family planning clinic .
	manualset3
127691	3	405725	13	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychosocial risk factors for obesity among women in a family planning clinic .
	manualset3
127692	4	405725	13	NULL	NULL	0	NULL	family planning clinic	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychosocial risk factors for obesity among women in a family planning clinic .
	manualset3
127693	1	405726	13	NULL	NULL	0	NULL	Public funds finance 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Public funds finance the prevention measures in its entirety .
	manualset3
127694	2	405726	13	NULL	NULL	0	NULL	prevention measures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Public funds finance the prevention measures in its entirety .
	manualset3
127695	3	405726	13	NULL	NULL	0	NULL	entirety 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Public funds finance the prevention measures in its entirety .
	manualset3
127696	1	405727	13	NULL	NULL	0	NULL	Pulmonary angiitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary angiitis and granulomatosis : a review .
	manualset3
127697	2	405727	13	NULL	NULL	0	NULL	granulomatosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary angiitis and granulomatosis : a review .
	manualset3
127698	3	405727	13	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary angiitis and granulomatosis : a review .
	manualset3
127699	1	405728	13	NULL	NULL	0	NULL	Pulmonary angiogenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary angiogenesis , mediated by the vascular endothelial growth factor ( VEGF ) pathway , is essential for alveolarization .
	manualset3
127700	2	405728	13	NULL	NULL	0	NULL	vascular endothelial growth factor ( VEGF ) pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary angiogenesis , mediated by the vascular endothelial growth factor ( VEGF ) pathway , is essential for alveolarization .
	manualset3
127701	3	405728	13	NULL	NULL	0	NULL	alveolarization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary angiogenesis , mediated by the vascular endothelial growth factor ( VEGF ) pathway , is essential for alveolarization .
	manualset3
127702	1	405729	13	NULL	NULL	0	NULL	man	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A man with a swollen tongue ) .
	manualset3
127703	2	405729	13	NULL	NULL	0	NULL	swollen tongue 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A man with a swollen tongue ) .
	manualset3
127704	1	405730	13	NULL	NULL	0	NULL	Pulmonary evaluation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary evaluation of permissible exposure limit of syntroleum S-8 synthetic jet fuel in mice .
	manualset3
127705	2	405730	13	NULL	NULL	0	NULL	permissible exposure limit 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary evaluation of permissible exposure limit of syntroleum S-8 synthetic jet fuel in mice .
	manualset3
127706	3	405730	13	NULL	NULL	0	NULL	syntroleum S-8 synthetic jet fuel	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary evaluation of permissible exposure limit of syntroleum S-8 synthetic jet fuel in mice .
	manualset3
127707	4	405730	13	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary evaluation of permissible exposure limit of syntroleum S-8 synthetic jet fuel in mice .
	manualset3
127708	1	405731	13	NULL	NULL	0	NULL	Pulmonary hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary hypertension is a survival-limiting complication in adults with homozygous sickle cell disease ( SS ) , but little is known about the development , course , or best treatment of pulmonary hypertension in children with SS .
	manualset3
127709	2	405731	13	NULL	NULL	0	NULL	survival-limiting complication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary hypertension is a survival-limiting complication in adults with homozygous sickle cell disease ( SS ) , but little is known about the development , course , or best treatment of pulmonary hypertension in children with SS .
	manualset3
127710	3	405731	13	NULL	NULL	0	NULL	adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary hypertension is a survival-limiting complication in adults with homozygous sickle cell disease ( SS ) , but little is known about the development , course , or best treatment of pulmonary hypertension in children with SS .
	manualset3
127711	4	405731	13	NULL	NULL	0	NULL	homozygous sickle cell disease ( SS )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary hypertension is a survival-limiting complication in adults with homozygous sickle cell disease ( SS ) , but little is known about the development , course , or best treatment of pulmonary hypertension in children with SS .
	manualset3
127712	5	405731	13	NULL	NULL	0	NULL	development	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary hypertension is a survival-limiting complication in adults with homozygous sickle cell disease ( SS ) , but little is known about the development , course , or best treatment of pulmonary hypertension in children with SS .
	manualset3
127713	6	405731	13	NULL	NULL	NULL	NULL	course	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pulmonary hypertension is a survival-limiting complication in adults with homozygous sickle cell disease ( SS ) , but little is known about the development , course , or best treatment of pulmonary hypertension in children with SS .
	manualset3
127714	7	405731	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary hypertension is a survival-limiting complication in adults with homozygous sickle cell disease ( SS ) , but little is known about the development , course , or best treatment of pulmonary hypertension in children with SS .
	manualset3
127715	8	405731	13	NULL	NULL	0	NULL	pulmonary hypertension 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary hypertension is a survival-limiting complication in adults with homozygous sickle cell disease ( SS ) , but little is known about the development , course , or best treatment of pulmonary hypertension in children with SS .
	manualset3
127716	9	405731	13	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary hypertension is a survival-limiting complication in adults with homozygous sickle cell disease ( SS ) , but little is known about the development , course , or best treatment of pulmonary hypertension in children with SS .
	manualset3
127717	10	405731	13	NULL	NULL	0	NULL	SS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary hypertension is a survival-limiting complication in adults with homozygous sickle cell disease ( SS ) , but little is known about the development , course , or best treatment of pulmonary hypertension in children with SS .
	manualset3
127718	1	405732	13	NULL	NULL	0	NULL	Pulmonary hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary hypertension was secondary in 41 patients with Eisenmenger 's syndrome , these comprising 27 females and 14 males aged 27.0 + / - 12.0 years , with a range from 4 through 51 years , and primary in the other 7 patients , 5 females and 2 males , whose age was 30.0 + / - 14.0 years , with a range from 9 through 52 years .
	manualset3
127719	2	405732	13	NULL	NULL	0	NULL	41 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary hypertension was secondary in 41 patients with Eisenmenger 's syndrome , these comprising 27 females and 14 males aged 27.0 + / - 12.0 years , with a range from 4 through 51 years , and primary in the other 7 patients , 5 females and 2 males , whose age was 30.0 + / - 14.0 years , with a range from 9 through 52 years .
	manualset3
127720	3	405732	13	NULL	NULL	0	NULL	Eisenmenger 's syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary hypertension was secondary in 41 patients with Eisenmenger 's syndrome , these comprising 27 females and 14 males aged 27.0 + / - 12.0 years , with a range from 4 through 51 years , and primary in the other 7 patients , 5 females and 2 males , whose age was 30.0 + / - 14.0 years , with a range from 9 through 52 years .
	manualset3
127721	4	405732	13	NULL	NULL	0	NULL	27 females	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary hypertension was secondary in 41 patients with Eisenmenger 's syndrome , these comprising 27 females and 14 males aged 27.0 + / - 12.0 years , with a range from 4 through 51 years , and primary in the other 7 patients , 5 females and 2 males , whose age was 30.0 + / - 14.0 years , with a range from 9 through 52 years .
	manualset3
127722	5	405732	13	NULL	NULL	0	NULL	14 males	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary hypertension was secondary in 41 patients with Eisenmenger 's syndrome , these comprising 27 females and 14 males aged 27.0 + / - 12.0 years , with a range from 4 through 51 years , and primary in the other 7 patients , 5 females and 2 males , whose age was 30.0 + / - 14.0 years , with a range from 9 through 52 years .
	manualset3
127723	6	405732	13	NULL	NULL	0	NULL	27.0 + / - 12.0 years	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary hypertension was secondary in 41 patients with Eisenmenger 's syndrome , these comprising 27 females and 14 males aged 27.0 + / - 12.0 years , with a range from 4 through 51 years , and primary in the other 7 patients , 5 females and 2 males , whose age was 30.0 + / - 14.0 years , with a range from 9 through 52 years .
	manualset3
127724	7	405732	13	NULL	NULL	0	NULL	range from 4	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary hypertension was secondary in 41 patients with Eisenmenger 's syndrome , these comprising 27 females and 14 males aged 27.0 + / - 12.0 years , with a range from 4 through 51 years , and primary in the other 7 patients , 5 females and 2 males , whose age was 30.0 + / - 14.0 years , with a range from 9 through 52 years .
	manualset3
127725	8	405732	13	NULL	NULL	0	NULL	51 years	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary hypertension was secondary in 41 patients with Eisenmenger 's syndrome , these comprising 27 females and 14 males aged 27.0 + / - 12.0 years , with a range from 4 through 51 years , and primary in the other 7 patients , 5 females and 2 males , whose age was 30.0 + / - 14.0 years , with a range from 9 through 52 years .
	manualset3
127726	9	405732	13	NULL	NULL	0	NULL	7 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary hypertension was secondary in 41 patients with Eisenmenger 's syndrome , these comprising 27 females and 14 males aged 27.0 + / - 12.0 years , with a range from 4 through 51 years , and primary in the other 7 patients , 5 females and 2 males , whose age was 30.0 + / - 14.0 years , with a range from 9 through 52 years .
	manualset3
127727	10	405732	13	NULL	NULL	0	NULL	5 females 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary hypertension was secondary in 41 patients with Eisenmenger 's syndrome , these comprising 27 females and 14 males aged 27.0 + / - 12.0 years , with a range from 4 through 51 years , and primary in the other 7 patients , 5 females and 2 males , whose age was 30.0 + / - 14.0 years , with a range from 9 through 52 years .
	manualset3
127728	11	405732	13	NULL	NULL	0	NULL	2 males	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary hypertension was secondary in 41 patients with Eisenmenger 's syndrome , these comprising 27 females and 14 males aged 27.0 + / - 12.0 years , with a range from 4 through 51 years , and primary in the other 7 patients , 5 females and 2 males , whose age was 30.0 + / - 14.0 years , with a range from 9 through 52 years .
	manualset3
127729	12	405732	13	NULL	NULL	0	NULL	age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary hypertension was secondary in 41 patients with Eisenmenger 's syndrome , these comprising 27 females and 14 males aged 27.0 + / - 12.0 years , with a range from 4 through 51 years , and primary in the other 7 patients , 5 females and 2 males , whose age was 30.0 + / - 14.0 years , with a range from 9 through 52 years .
	manualset3
127730	13	405732	13	NULL	NULL	0	NULL	30.0 + / - 14.0 years	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary hypertension was secondary in 41 patients with Eisenmenger 's syndrome , these comprising 27 females and 14 males aged 27.0 + / - 12.0 years , with a range from 4 through 51 years , and primary in the other 7 patients , 5 females and 2 males , whose age was 30.0 + / - 14.0 years , with a range from 9 through 52 years .
	manualset3
127731	14	405732	13	NULL	NULL	0	NULL	range from 9 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary hypertension was secondary in 41 patients with Eisenmenger 's syndrome , these comprising 27 females and 14 males aged 27.0 + / - 12.0 years , with a range from 4 through 51 years , and primary in the other 7 patients , 5 females and 2 males , whose age was 30.0 + / - 14.0 years , with a range from 9 through 52 years .
	manualset3
127732	15	405732	13	NULL	NULL	0	NULL	52 years	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary hypertension was secondary in 41 patients with Eisenmenger 's syndrome , these comprising 27 females and 14 males aged 27.0 + / - 12.0 years , with a range from 4 through 51 years , and primary in the other 7 patients , 5 females and 2 males , whose age was 30.0 + / - 14.0 years , with a range from 9 through 52 years .
	manualset3
127733	1	405733	13	NULL	NULL	0	NULL	Pulmonary perfusion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary perfusion was successfully but temporarily restored by the intervention .
	manualset3
127734	2	405733	13	NULL	NULL	0	NULL	intervention 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary perfusion was successfully but temporarily restored by the intervention .
	manualset3
127735	1	405734	13	NULL	NULL	0	NULL	Pulmonary scintigraphy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary scintigraphy is a key investigation in the diagnosis of PE due to its innocuity and high sensitivity .
	manualset3
127736	2	405734	13	NULL	NULL	0	NULL	investigation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary scintigraphy is a key investigation in the diagnosis of PE due to its innocuity and high sensitivity .
	manualset3
127737	3	405734	13	NULL	NULL	NULL	NULL	diagnosis	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pulmonary scintigraphy is a key investigation in the diagnosis of PE due to its innocuity and high sensitivity .
	manualset3
127738	4	405734	13	NULL	NULL	0	NULL	PE	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary scintigraphy is a key investigation in the diagnosis of PE due to its innocuity and high sensitivity .
	manualset3
127739	5	405734	13	NULL	NULL	0	NULL	innocuity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary scintigraphy is a key investigation in the diagnosis of PE due to its innocuity and high sensitivity .
	manualset3
127740	6	405734	13	NULL	NULL	0	NULL	high sensitivity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary scintigraphy is a key investigation in the diagnosis of PE due to its innocuity and high sensitivity .
	manualset3
127741	1	405735	13	NULL	NULL	0	NULL	Pulmonary sequestration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary sequestration : an aberrant systemic blood supply demonstrated by computed tomographic angiography with 3-dimensional reconstruction .
	manualset3
127742	2	405735	13	NULL	NULL	0	NULL	aberrant systemic blood supply	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary sequestration : an aberrant systemic blood supply demonstrated by computed tomographic angiography with 3-dimensional reconstruction .
	manualset3
127743	3	405735	13	NULL	NULL	0	NULL	computed tomographic angiography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary sequestration : an aberrant systemic blood supply demonstrated by computed tomographic angiography with 3-dimensional reconstruction .
	manualset3
127744	4	405735	13	NULL	NULL	0	NULL	3-dimensional reconstruction	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary sequestration : an aberrant systemic blood supply demonstrated by computed tomographic angiography with 3-dimensional reconstruction .
	manualset3
127745	1	405736	13	NULL	NULL	0	NULL	Pulmonary thromboembolism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary thromboembolism during adult liver transplantation : incidence , clinical presentation , outcome , risk factors , and diagnostic predictors .
	manualset3
127746	2	405736	13	NULL	NULL	0	NULL	adult liver transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary thromboembolism during adult liver transplantation : incidence , clinical presentation , outcome , risk factors , and diagnostic predictors .
	manualset3
127747	3	405736	13	NULL	NULL	0	NULL	incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary thromboembolism during adult liver transplantation : incidence , clinical presentation , outcome , risk factors , and diagnostic predictors .
	manualset3
127748	4	405736	13	NULL	NULL	0	NULL	clinical presentation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary thromboembolism during adult liver transplantation : incidence , clinical presentation , outcome , risk factors , and diagnostic predictors .
	manualset3
127749	5	405736	13	NULL	NULL	0	NULL	outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary thromboembolism during adult liver transplantation : incidence , clinical presentation , outcome , risk factors , and diagnostic predictors .
	manualset3
127750	6	405736	13	NULL	NULL	0	NULL	risk factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary thromboembolism during adult liver transplantation : incidence , clinical presentation , outcome , risk factors , and diagnostic predictors .
	manualset3
127751	7	405736	13	NULL	NULL	0	NULL	diagnostic predictors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary thromboembolism during adult liver transplantation : incidence , clinical presentation , outcome , risk factors , and diagnostic predictors .
	manualset3
127752	1	405737	13	NULL	NULL	0	NULL	Pulmonary ultrastructure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary ultrastructure and systemic fibrinolysis .
	manualset3
127753	2	405737	13	NULL	NULL	0	NULL	systemic fibrinolysis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary ultrastructure and systemic fibrinolysis .
	manualset3
127754	1	405738	13	NULL	NULL	0	NULL	Pulsatile cardiopulmonary bypass ( CPB )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulsatile cardiopulmonary bypass ( CPB ) has been suggested to be superior to nonpulsatile CPB .
	manualset3
127755	2	405738	13	NULL	NULL	0	NULL	nonpulsatile CPB	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulsatile cardiopulmonary bypass ( CPB ) has been suggested to be superior to nonpulsatile CPB .
	manualset3
127756	1	405739	13	NULL	NULL	0	NULL	man	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A man with no previous history of allergy or chest disease developed asthma after exposure to a heavy atmospheric concentration of amprolium hydrochloride which is a constituent of a poultry-food additive .
	manualset3
127757	2	405739	13	NULL	NULL	0	NULL	previous history of allergy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A man with no previous history of allergy or chest disease developed asthma after exposure to a heavy atmospheric concentration of amprolium hydrochloride which is a constituent of a poultry-food additive .
	manualset3
127758	3	405739	13	NULL	NULL	0	NULL	chest disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A man with no previous history of allergy or chest disease developed asthma after exposure to a heavy atmospheric concentration of amprolium hydrochloride which is a constituent of a poultry-food additive .
	manualset3
127759	4	405739	13	NULL	NULL	0	NULL	asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A man with no previous history of allergy or chest disease developed asthma after exposure to a heavy atmospheric concentration of amprolium hydrochloride which is a constituent of a poultry-food additive .
	manualset3
127760	5	405739	13	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A man with no previous history of allergy or chest disease developed asthma after exposure to a heavy atmospheric concentration of amprolium hydrochloride which is a constituent of a poultry-food additive .
	manualset3
127761	6	405739	13	NULL	NULL	0	NULL	heavy atmospheric concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A man with no previous history of allergy or chest disease developed asthma after exposure to a heavy atmospheric concentration of amprolium hydrochloride which is a constituent of a poultry-food additive .
	manualset3
127762	7	405739	13	NULL	NULL	0	NULL	amprolium hydrochloride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A man with no previous history of allergy or chest disease developed asthma after exposure to a heavy atmospheric concentration of amprolium hydrochloride which is a constituent of a poultry-food additive .
	manualset3
127763	8	405739	13	NULL	NULL	0	NULL	constituent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A man with no previous history of allergy or chest disease developed asthma after exposure to a heavy atmospheric concentration of amprolium hydrochloride which is a constituent of a poultry-food additive .
	manualset3
127764	9	405739	13	NULL	NULL	NULL	NULL	poultry-food additive	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A man with no previous history of allergy or chest disease developed asthma after exposure to a heavy atmospheric concentration of amprolium hydrochloride which is a constituent of a poultry-food additive .
	manualset3
127765	1	405740	13	NULL	NULL	NULL	NULL	Pulsed-field gel electrophoresis patterns	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pulsed-field gel electrophoresis patterns of DNA digested with MluI included the specific B. burgdorferi sensu stricto band at 135 kbp for the five OspA-negative isolates from I. scapularis ticks .
	manualset3
127767	3	405740	13	NULL	NULL	0	NULL	DNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulsed-field gel electrophoresis patterns of DNA digested with MluI included the specific B. burgdorferi sensu stricto band at 135 kbp for the five OspA-negative isolates from I. scapularis ticks .
	manualset3
127768	4	405740	13	NULL	NULL	0	NULL	MluI	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulsed-field gel electrophoresis patterns of DNA digested with MluI included the specific B. burgdorferi sensu stricto band at 135 kbp for the five OspA-negative isolates from I. scapularis ticks .
	manualset3
127769	5	405740	13	NULL	NULL	0	NULL	B. burgdorferi sensu stricto	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulsed-field gel electrophoresis patterns of DNA digested with MluI included the specific B. burgdorferi sensu stricto band at 135 kbp for the five OspA-negative isolates from I. scapularis ticks .
	manualset3
127770	6	405740	13	NULL	NULL	0	NULL	band	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulsed-field gel electrophoresis patterns of DNA digested with MluI included the specific B. burgdorferi sensu stricto band at 135 kbp for the five OspA-negative isolates from I. scapularis ticks .
	manualset3
127771	7	405740	13	NULL	NULL	0	NULL	135 kbp	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulsed-field gel electrophoresis patterns of DNA digested with MluI included the specific B. burgdorferi sensu stricto band at 135 kbp for the five OspA-negative isolates from I. scapularis ticks .
	manualset3
127772	8	405740	13	NULL	NULL	0	NULL	five OspA-negative isolates	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulsed-field gel electrophoresis patterns of DNA digested with MluI included the specific B. burgdorferi sensu stricto band at 135 kbp for the five OspA-negative isolates from I. scapularis ticks .
	manualset3
127773	9	405740	13	NULL	NULL	0	NULL	I. scapularis ticks 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulsed-field gel electrophoresis patterns of DNA digested with MluI included the specific B. burgdorferi sensu stricto band at 135 kbp for the five OspA-negative isolates from I. scapularis ticks .
	manualset3
127774	1	405741	13	NULL	NULL	0	NULL	Pulses	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulses of increasing duration from 5-30 seconds promoted increased accumulation of 45Ca2 + ; intermittent 5 sec pulses , at 10-minute intervals , produced a stepwise accumulation of 45Ca2 + .
	manualset3
127775	2	405741	13	NULL	NULL	0	NULL	duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulses of increasing duration from 5-30 seconds promoted increased accumulation of 45Ca2 + ; intermittent 5 sec pulses , at 10-minute intervals , produced a stepwise accumulation of 45Ca2 + .
	manualset3
127776	3	405741	13	NULL	NULL	0	NULL	5-30 seconds	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulses of increasing duration from 5-30 seconds promoted increased accumulation of 45Ca2 + ; intermittent 5 sec pulses , at 10-minute intervals , produced a stepwise accumulation of 45Ca2 + .
	manualset3
127777	4	405741	13	NULL	NULL	0	NULL	accumulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulses of increasing duration from 5-30 seconds promoted increased accumulation of 45Ca2 + ; intermittent 5 sec pulses , at 10-minute intervals , produced a stepwise accumulation of 45Ca2 + .
	manualset3
127779	5	405741	13	NULL	NULL	0	NULL	45Ca2 + 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulses of increasing duration from 5-30 seconds promoted increased accumulation of 45Ca2 + ; intermittent 5 sec pulses , at 10-minute intervals , produced a stepwise accumulation of 45Ca2 + .
	manualset3
127780	6	405741	13	NULL	NULL	0	NULL	5 sec pulses	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulses of increasing duration from 5-30 seconds promoted increased accumulation of 45Ca2 + ; intermittent 5 sec pulses , at 10-minute intervals , produced a stepwise accumulation of 45Ca2 + .
	manualset3
127781	7	405741	13	NULL	NULL	0	NULL	10-minute intervals 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulses of increasing duration from 5-30 seconds promoted increased accumulation of 45Ca2 + ; intermittent 5 sec pulses , at 10-minute intervals , produced a stepwise accumulation of 45Ca2 + .
	manualset3
127782	8	405741	13	NULL	NULL	0	NULL	stepwise accumulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulses of increasing duration from 5-30 seconds promoted increased accumulation of 45Ca2 + ; intermittent 5 sec pulses , at 10-minute intervals , produced a stepwise accumulation of 45Ca2 + .
	manualset3
127783	9	405741	13	NULL	NULL	0	NULL	45Ca2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulses of increasing duration from 5-30 seconds promoted increased accumulation of 45Ca2 + ; intermittent 5 sec pulses , at 10-minute intervals , produced a stepwise accumulation of 45Ca2 + .
	manualset3
127784	1	405742	13	NULL	NULL	0	NULL	Pure cutaneous stimulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pure cutaneous stimulation provoked no effects on the motor-unit firing .
	manualset3
127785	2	405742	13	NULL	NULL	NULL	NULL	effects	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pure cutaneous stimulation provoked no effects on the motor-unit firing .
	manualset3
127786	3	405742	13	NULL	NULL	0	NULL	motor-unit firing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pure cutaneous stimulation provoked no effects on the motor-unit firing .
	manualset3
127787	1	405743	13	NULL	NULL	0	NULL	Purification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification and characterization of a protease produced by Bacillus megaterium RRM2 : application in detergent and dehairing industries .
	manualset3
127788	2	405743	13	NULL	NULL	0	NULL	characterization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification and characterization of a protease produced by Bacillus megaterium RRM2 : application in detergent and dehairing industries .
	manualset3
127789	3	405743	13	NULL	NULL	0	NULL	protease	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification and characterization of a protease produced by Bacillus megaterium RRM2 : application in detergent and dehairing industries .
	manualset3
127790	4	405743	13	NULL	NULL	0	NULL	Bacillus megaterium RRM2 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification and characterization of a protease produced by Bacillus megaterium RRM2 : application in detergent and dehairing industries .
	manualset3
127791	5	405743	13	NULL	NULL	0	NULL	application 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification and characterization of a protease produced by Bacillus megaterium RRM2 : application in detergent and dehairing industries .
	manualset3
127792	6	405743	13	NULL	NULL	NULL	NULL	detergent industries	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Purification and characterization of a protease produced by Bacillus megaterium RRM2 : application in detergent and dehairing industries .
	manualset3
127793	7	405743	13	NULL	NULL	0	NULL	dehairing industries	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification and characterization of a protease produced by Bacillus megaterium RRM2 : application in detergent and dehairing industries .
	manualset3
127794	1	405744	13	NULL	NULL	0	NULL	Purification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification and characterization of cystathionine gamma-lyase from Lactobacillus fermentum DT41 .
	manualset3
127795	2	405744	13	NULL	NULL	0	NULL	characterization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification and characterization of cystathionine gamma-lyase from Lactobacillus fermentum DT41 .
	manualset3
127796	3	405744	13	NULL	NULL	0	NULL	cystathionine gamma-lyase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification and characterization of cystathionine gamma-lyase from Lactobacillus fermentum DT41 .
	manualset3
127797	4	405744	13	NULL	NULL	0	NULL	Lactobacillus fermentum DT41 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification and characterization of cystathionine gamma-lyase from Lactobacillus fermentum DT41 .
	manualset3
127798	1	405745	13	NULL	NULL	0	NULL	Purification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification and characterization of fatty acid cyclooxygenase from human platelets .
	manualset3
127799	2	405745	13	NULL	NULL	0	NULL	characterization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification and characterization of fatty acid cyclooxygenase from human platelets .
	manualset3
127800	3	405745	13	NULL	NULL	0	NULL	fatty acid cyclooxygenase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification and characterization of fatty acid cyclooxygenase from human platelets .
	manualset3
127801	4	405745	13	NULL	NULL	0	NULL	human platelets 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification and characterization of fatty acid cyclooxygenase from human platelets .
	manualset3
127802	1	405746	13	NULL	NULL	0	NULL	Purification 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification and microsequencing of p68 showed that it was related to the previously described GAP-associated protein p62 ( ref .
	manualset3
127803	2	405746	13	NULL	NULL	0	NULL	microsequencing 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification and microsequencing of p68 showed that it was related to the previously described GAP-associated protein p62 ( ref .
	manualset3
127804	3	405746	13	NULL	NULL	0	NULL	p68 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification and microsequencing of p68 showed that it was related to the previously described GAP-associated protein p62 ( ref .
	manualset3
127805	4	405746	13	NULL	NULL	0	NULL	GAP-associated protein p62	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification and microsequencing of p68 showed that it was related to the previously described GAP-associated protein p62 ( ref .
	manualset3
127806	1	405747	13	NULL	NULL	0	NULL	Purification 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification and properties of extracellular glucosyltransferase from Streptococcus bovis .
	manualset3
127807	2	405747	13	NULL	NULL	0	NULL	properties 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification and properties of extracellular glucosyltransferase from Streptococcus bovis .
	manualset3
127808	3	405747	13	NULL	NULL	0	NULL	extracellular glucosyltransferase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification and properties of extracellular glucosyltransferase from Streptococcus bovis .
	manualset3
127809	4	405747	13	NULL	NULL	0	NULL	Streptococcus bovis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification and properties of extracellular glucosyltransferase from Streptococcus bovis .
	manualset3
127810	1	405748	13	NULL	NULL	0	NULL	Purification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification and some properties of alpha-L-arabinofuranosidase from Bacillus subtilis 3-6 .
	manualset3
127811	2	405748	13	NULL	NULL	0	NULL	properties	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification and some properties of alpha-L-arabinofuranosidase from Bacillus subtilis 3-6 .
	manualset3
127812	3	405748	13	NULL	NULL	0	NULL	alpha-L-arabinofuranosidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification and some properties of alpha-L-arabinofuranosidase from Bacillus subtilis 3-6 .
	manualset3
127813	4	405748	13	NULL	NULL	0	NULL	Bacillus subtilis 3-6 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification and some properties of alpha-L-arabinofuranosidase from Bacillus subtilis 3-6 .
	manualset3
127814	1	405749	13	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A mandatory role for STAT4 in IL-12 induction of mouse T cell CCR5 .
	manualset3
127815	2	405749	13	NULL	NULL	0	NULL	STAT4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A mandatory role for STAT4 in IL-12 induction of mouse T cell CCR5 .
	manualset3
127816	3	405749	13	NULL	NULL	0	NULL	IL-12 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A mandatory role for STAT4 in IL-12 induction of mouse T cell CCR5 .
	manualset3
127817	4	405749	13	NULL	NULL	0	NULL	induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A mandatory role for STAT4 in IL-12 induction of mouse T cell CCR5 .
	manualset3
127818	5	405749	13	NULL	NULL	NULL	NULL	mouse T cell CCR5 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A mandatory role for STAT4 in IL-12 induction of mouse T cell CCR5 .
	manualset3
127820	1	405750	13	NULL	NULL	0	NULL	Purification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification of a putative Na + / D-glucose cotransporter from pig kidney brush border membranes on a phlorizin affinity column .
	manualset3
127821	2	405750	13	NULL	NULL	0	NULL	putative Na + / D-glucose cotransporter	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification of a putative Na + / D-glucose cotransporter from pig kidney brush border membranes on a phlorizin affinity column .
	manualset3
127822	3	405750	13	NULL	NULL	0	NULL	pig kidney brush border membranes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification of a putative Na + / D-glucose cotransporter from pig kidney brush border membranes on a phlorizin affinity column .
	manualset3
127823	4	405750	13	NULL	NULL	0	NULL	phlorizin affinity column 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification of a putative Na + / D-glucose cotransporter from pig kidney brush border membranes on a phlorizin affinity column .
	manualset3
127824	1	405751	13	NULL	NULL	0	NULL	Purification 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification of bacterial cytochrome P-450 .
	manualset3
127825	2	405751	13	NULL	NULL	0	NULL	bacterial cytochrome P-450	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification of bacterial cytochrome P-450 .
	manualset3
127826	1	405752	13	NULL	NULL	0	NULL	Purification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification of monoclonal antibodies from tissue culture medium depleted of IgG .
	manualset3
127827	2	405752	13	NULL	NULL	0	NULL	monoclonal antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification of monoclonal antibodies from tissue culture medium depleted of IgG .
	manualset3
127828	3	405752	13	NULL	NULL	0	NULL	tissue culture medium 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification of monoclonal antibodies from tissue culture medium depleted of IgG .
	manualset3
127829	4	405752	13	NULL	NULL	0	NULL	IgG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification of monoclonal antibodies from tissue culture medium depleted of IgG .
	manualset3
127830	1	405753	13	NULL	NULL	0	NULL	Purification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification of pox viruses by density gradient centrifugation .
	manualset3
127831	2	405753	13	NULL	NULL	0	NULL	pox viruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification of pox viruses by density gradient centrifugation .
	manualset3
127832	3	405753	13	NULL	NULL	0	NULL	density gradient centrifugation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification of pox viruses by density gradient centrifugation .
	manualset3
127833	1	405754	13	NULL	NULL	0	NULL	GEFs 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Purified GEFs ( the catalytic domain of yeast Sdc25p and the full-length and catalytic domain of mouse CDC25Mm ) and the Ras binding domains ( RBDs ) of Raf-1 ( Raf ( 1-149 ) and Raf ( 51-131 ) ) were used .
	manualset3
127834	2	405754	13	NULL	NULL	NULL	NULL	catalytic domain of yeast Sdc25p	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Purified GEFs ( the catalytic domain of yeast Sdc25p and the full-length and catalytic domain of mouse CDC25Mm ) and the Ras binding domains ( RBDs ) of Raf-1 ( Raf ( 1-149 ) and Raf ( 51-131 ) ) were used .
	manualset3
127836	4	405754	13	NULL	NULL	0	NULL	full-length mouse CDC25Mm	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Purified GEFs ( the catalytic domain of yeast Sdc25p and the full-length and catalytic domain of mouse CDC25Mm ) and the Ras binding domains ( RBDs ) of Raf-1 ( Raf ( 1-149 ) and Raf ( 51-131 ) ) were used .
	manualset3
127837	5	405754	13	NULL	NULL	0	NULL	catalytic domain of mouse CDC25Mm	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Purified GEFs ( the catalytic domain of yeast Sdc25p and the full-length and catalytic domain of mouse CDC25Mm ) and the Ras binding domains ( RBDs ) of Raf-1 ( Raf ( 1-149 ) and Raf ( 51-131 ) ) were used .
	manualset3
127838	6	405754	13	NULL	NULL	0	NULL	Ras binding domains ( RBDs ) of Raf-1 ( Raf ( 1-149 ) 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Purified GEFs ( the catalytic domain of yeast Sdc25p and the full-length and catalytic domain of mouse CDC25Mm ) and the Ras binding domains ( RBDs ) of Raf-1 ( Raf ( 1-149 ) and Raf ( 51-131 ) ) were used .
	manualset3
127839	7	405754	13	NULL	NULL	0	NULL	Ras binding domains ( RBDs ) of Raf-1 (Raf ( 51-131 ) ) 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Purified GEFs ( the catalytic domain of yeast Sdc25p and the full-length and catalytic domain of mouse CDC25Mm ) and the Ras binding domains ( RBDs ) of Raf-1 ( Raf ( 1-149 ) and Raf ( 51-131 ) ) were used .
	manualset3
127840	1	405755	13	NULL	NULL	0	NULL	GP 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Purified GP was shown to exhibit a weak , but significant , acid phosphatase activity by hydrolyzing alpha-naphthyl phosphate at pH 5.6 .
	manualset3
127841	2	405755	13	NULL	NULL	0	NULL	acid phosphatase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Purified GP was shown to exhibit a weak , but significant , acid phosphatase activity by hydrolyzing alpha-naphthyl phosphate at pH 5.6 .
	manualset3
127842	3	405755	13	NULL	NULL	0	NULL	alpha-naphthyl phosphate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Purified GP was shown to exhibit a weak , but significant , acid phosphatase activity by hydrolyzing alpha-naphthyl phosphate at pH 5.6 .
	manualset3
127843	4	405755	13	NULL	NULL	0	NULL	pH 5.6	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Purified GP was shown to exhibit a weak , but significant , acid phosphatase activity by hydrolyzing alpha-naphthyl phosphate at pH 5.6 .
	manualset3
127844	1	405756	13	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Purified protein was used to investigate the nature of its interaction with membranes and with Ca2 + .
	manualset3
127845	2	405756	13	NULL	NULL	0	NULL	nature	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Purified protein was used to investigate the nature of its interaction with membranes and with Ca2 + .
	manualset3
127846	3	405756	13	NULL	NULL	0	NULL	interaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Purified protein was used to investigate the nature of its interaction with membranes and with Ca2 + .
	manualset3
127847	4	405756	13	NULL	NULL	0	NULL	membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Purified protein was used to investigate the nature of its interaction with membranes and with Ca2 + .
	manualset3
127848	5	405756	13	NULL	NULL	0	NULL	Ca2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Purified protein was used to investigate the nature of its interaction with membranes and with Ca2 + .
	manualset3
127849	1	405757	13	NULL	NULL	0	NULL	virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Purified virus and procapsids were obtained by treating the infected cytoplasmic extracts with RNase and EDTA .
	manualset3
127850	2	405757	13	NULL	NULL	0	NULL	procapsids 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Purified virus and procapsids were obtained by treating the infected cytoplasmic extracts with RNase and EDTA .
	manualset3
127851	3	405757	13	NULL	NULL	0	NULL	cytoplasmic extracts	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Purified virus and procapsids were obtained by treating the infected cytoplasmic extracts with RNase and EDTA .
	manualset3
127852	4	405757	13	NULL	NULL	0	NULL	RNase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Purified virus and procapsids were obtained by treating the infected cytoplasmic extracts with RNase and EDTA .
	manualset3
127853	5	405757	13	NULL	NULL	0	NULL	EDTA 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Purified virus and procapsids were obtained by treating the infected cytoplasmic extracts with RNase and EDTA .
	manualset3
127854	1	405758	13	NULL	NULL	0	NULL	decrease 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A marked decrease in enzyme content occurred in late gestation and was maintained throughout lactation ; upon weaning , the enzyme content returned to the levels found in virgin mice .
	manualset3
127855	2	405758	13	NULL	NULL	0	NULL	enzyme 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A marked decrease in enzyme content occurred in late gestation and was maintained throughout lactation ; upon weaning , the enzyme content returned to the levels found in virgin mice .
	manualset3
127856	3	405758	13	NULL	NULL	0	NULL	content	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A marked decrease in enzyme content occurred in late gestation and was maintained throughout lactation ; upon weaning , the enzyme content returned to the levels found in virgin mice .
	manualset3
127857	4	405758	13	NULL	NULL	0	NULL	late gestation	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A marked decrease in enzyme content occurred in late gestation and was maintained throughout lactation ; upon weaning , the enzyme content returned to the levels found in virgin mice .
	manualset3
127858	5	405758	13	NULL	NULL	0	NULL	lactation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A marked decrease in enzyme content occurred in late gestation and was maintained throughout lactation ; upon weaning , the enzyme content returned to the levels found in virgin mice .
	manualset3
127859	6	405758	13	NULL	NULL	0	NULL	enzyme 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A marked decrease in enzyme content occurred in late gestation and was maintained throughout lactation ; upon weaning , the enzyme content returned to the levels found in virgin mice .
	manualset3
127860	7	405758	13	NULL	NULL	0	NULL	content 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A marked decrease in enzyme content occurred in late gestation and was maintained throughout lactation ; upon weaning , the enzyme content returned to the levels found in virgin mice .
	manualset3
127861	8	405758	13	NULL	NULL	0	NULL	levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A marked decrease in enzyme content occurred in late gestation and was maintained throughout lactation ; upon weaning , the enzyme content returned to the levels found in virgin mice .
	manualset3
127862	9	405758	13	NULL	NULL	0	NULL	virgin mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A marked decrease in enzyme content occurred in late gestation and was maintained throughout lactation ; upon weaning , the enzyme content returned to the levels found in virgin mice .
	manualset3
127863	1	405759	13	NULL	NULL	0	NULL	Purpose 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : The aim of the study was to assess the concentration of chemokines : CXCL10 , XCL11 , CXCL12 , CXCL13 in serum and cerebrospinal fluid ( CSF ) in patients with tick-borne encephalitis ( TBE ) before and after treatment .
	manualset3
127864	2	405759	13	NULL	NULL	0	NULL	aim	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : The aim of the study was to assess the concentration of chemokines : CXCL10 , XCL11 , CXCL12 , CXCL13 in serum and cerebrospinal fluid ( CSF ) in patients with tick-borne encephalitis ( TBE ) before and after treatment .
	manualset3
127865	3	405759	13	NULL	NULL	NULL	NULL	study 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Purpose : The aim of the study was to assess the concentration of chemokines : CXCL10 , XCL11 , CXCL12 , CXCL13 in serum and cerebrospinal fluid ( CSF ) in patients with tick-borne encephalitis ( TBE ) before and after treatment .
	manualset3
127866	4	405759	13	NULL	NULL	0	NULL	concentration 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : The aim of the study was to assess the concentration of chemokines : CXCL10 , XCL11 , CXCL12 , CXCL13 in serum and cerebrospinal fluid ( CSF ) in patients with tick-borne encephalitis ( TBE ) before and after treatment .
	manualset3
127867	5	405759	13	NULL	NULL	0	NULL	chemokines 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : The aim of the study was to assess the concentration of chemokines : CXCL10 , XCL11 , CXCL12 , CXCL13 in serum and cerebrospinal fluid ( CSF ) in patients with tick-borne encephalitis ( TBE ) before and after treatment .
	manualset3
127868	6	405759	13	NULL	NULL	0	NULL	CXCL10 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : The aim of the study was to assess the concentration of chemokines : CXCL10 , XCL11 , CXCL12 , CXCL13 in serum and cerebrospinal fluid ( CSF ) in patients with tick-borne encephalitis ( TBE ) before and after treatment .
	manualset3
127869	7	405759	13	NULL	NULL	0	NULL	XCL11 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : The aim of the study was to assess the concentration of chemokines : CXCL10 , XCL11 , CXCL12 , CXCL13 in serum and cerebrospinal fluid ( CSF ) in patients with tick-borne encephalitis ( TBE ) before and after treatment .
	manualset3
127870	8	405759	13	NULL	NULL	0	NULL	CXCL12 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : The aim of the study was to assess the concentration of chemokines : CXCL10 , XCL11 , CXCL12 , CXCL13 in serum and cerebrospinal fluid ( CSF ) in patients with tick-borne encephalitis ( TBE ) before and after treatment .
	manualset3
127871	9	405759	13	NULL	NULL	0	NULL	CXCL13 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : The aim of the study was to assess the concentration of chemokines : CXCL10 , XCL11 , CXCL12 , CXCL13 in serum and cerebrospinal fluid ( CSF ) in patients with tick-borne encephalitis ( TBE ) before and after treatment .
	manualset3
127872	10	405759	13	NULL	NULL	0	NULL	serum 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : The aim of the study was to assess the concentration of chemokines : CXCL10 , XCL11 , CXCL12 , CXCL13 in serum and cerebrospinal fluid ( CSF ) in patients with tick-borne encephalitis ( TBE ) before and after treatment .
	manualset3
127873	11	405759	13	NULL	NULL	0	NULL	cerebrospinal fluid ( CSF )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : The aim of the study was to assess the concentration of chemokines : CXCL10 , XCL11 , CXCL12 , CXCL13 in serum and cerebrospinal fluid ( CSF ) in patients with tick-borne encephalitis ( TBE ) before and after treatment .
	manualset3
127874	12	405759	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : The aim of the study was to assess the concentration of chemokines : CXCL10 , XCL11 , CXCL12 , CXCL13 in serum and cerebrospinal fluid ( CSF ) in patients with tick-borne encephalitis ( TBE ) before and after treatment .
	manualset3
127875	13	405759	13	NULL	NULL	0	NULL	tick-borne encephalitis ( TBE ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : The aim of the study was to assess the concentration of chemokines : CXCL10 , XCL11 , CXCL12 , CXCL13 in serum and cerebrospinal fluid ( CSF ) in patients with tick-borne encephalitis ( TBE ) before and after treatment .
	manualset3
127876	14	405759	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : The aim of the study was to assess the concentration of chemokines : CXCL10 , XCL11 , CXCL12 , CXCL13 in serum and cerebrospinal fluid ( CSF ) in patients with tick-borne encephalitis ( TBE ) before and after treatment .
	manualset3
127877	1	405760	13	NULL	NULL	0	NULL	Purpose	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : To investigate the effects of intravitreal ranibizumab on retrobulbar blood flow in patients with neovascular age-related macular degeneration ( AMD ) .
	manualset3
127878	2	405760	13	NULL	NULL	0	NULL	effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : To investigate the effects of intravitreal ranibizumab on retrobulbar blood flow in patients with neovascular age-related macular degeneration ( AMD ) .
	manualset3
127879	3	405760	13	NULL	NULL	0	NULL	intravitreal ranibizumab	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : To investigate the effects of intravitreal ranibizumab on retrobulbar blood flow in patients with neovascular age-related macular degeneration ( AMD ) .
	manualset3
127880	4	405760	13	NULL	NULL	0	NULL	retrobulbar blood flow	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : To investigate the effects of intravitreal ranibizumab on retrobulbar blood flow in patients with neovascular age-related macular degeneration ( AMD ) .
	manualset3
127881	5	405760	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : To investigate the effects of intravitreal ranibizumab on retrobulbar blood flow in patients with neovascular age-related macular degeneration ( AMD ) .
	manualset3
127882	6	405760	13	NULL	NULL	0	NULL	neovascular age-related macular degeneration ( AMD )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : To investigate the effects of intravitreal ranibizumab on retrobulbar blood flow in patients with neovascular age-related macular degeneration ( AMD ) .
	manualset3
127883	1	405761	13	NULL	NULL	0	NULL	Purpose 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : We aimed to investigate whether test performance in neurological and cognitive areas is able to predict daily task performance in stroke patients and if the two selected measures of stroke severity and cognitive function could be used as valid tools to predict functional outcomes after stroke .
	manualset3
127884	2	405761	13	NULL	NULL	0	NULL	test performance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : We aimed to investigate whether test performance in neurological and cognitive areas is able to predict daily task performance in stroke patients and if the two selected measures of stroke severity and cognitive function could be used as valid tools to predict functional outcomes after stroke .
	manualset3
127885	3	405761	13	NULL	NULL	0	NULL	neurological areas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : We aimed to investigate whether test performance in neurological and cognitive areas is able to predict daily task performance in stroke patients and if the two selected measures of stroke severity and cognitive function could be used as valid tools to predict functional outcomes after stroke .
	manualset3
127886	4	405761	13	NULL	NULL	0	NULL	cognitive areas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : We aimed to investigate whether test performance in neurological and cognitive areas is able to predict daily task performance in stroke patients and if the two selected measures of stroke severity and cognitive function could be used as valid tools to predict functional outcomes after stroke .
	manualset3
127887	5	405761	13	NULL	NULL	0	NULL	task performance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : We aimed to investigate whether test performance in neurological and cognitive areas is able to predict daily task performance in stroke patients and if the two selected measures of stroke severity and cognitive function could be used as valid tools to predict functional outcomes after stroke .
	manualset3
127888	6	405761	13	NULL	NULL	0	NULL	stroke patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : We aimed to investigate whether test performance in neurological and cognitive areas is able to predict daily task performance in stroke patients and if the two selected measures of stroke severity and cognitive function could be used as valid tools to predict functional outcomes after stroke .
	manualset3
127889	7	405761	13	NULL	NULL	0	NULL	two selected measures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : We aimed to investigate whether test performance in neurological and cognitive areas is able to predict daily task performance in stroke patients and if the two selected measures of stroke severity and cognitive function could be used as valid tools to predict functional outcomes after stroke .
	manualset3
127890	8	405761	13	NULL	NULL	0	NULL	stroke severity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : We aimed to investigate whether test performance in neurological and cognitive areas is able to predict daily task performance in stroke patients and if the two selected measures of stroke severity and cognitive function could be used as valid tools to predict functional outcomes after stroke .
	manualset3
127891	9	405761	13	NULL	NULL	0	NULL	cognitive function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : We aimed to investigate whether test performance in neurological and cognitive areas is able to predict daily task performance in stroke patients and if the two selected measures of stroke severity and cognitive function could be used as valid tools to predict functional outcomes after stroke .
	manualset3
127892	10	405761	13	NULL	NULL	0	NULL	valid tools	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : We aimed to investigate whether test performance in neurological and cognitive areas is able to predict daily task performance in stroke patients and if the two selected measures of stroke severity and cognitive function could be used as valid tools to predict functional outcomes after stroke .
	manualset3
127893	11	405761	13	NULL	NULL	0	NULL	functional outcomes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : We aimed to investigate whether test performance in neurological and cognitive areas is able to predict daily task performance in stroke patients and if the two selected measures of stroke severity and cognitive function could be used as valid tools to predict functional outcomes after stroke .
	manualset3
127894	12	405761	13	NULL	NULL	0	NULL	stroke 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Purpose : We aimed to investigate whether test performance in neurological and cognitive areas is able to predict daily task performance in stroke patients and if the two selected measures of stroke severity and cognitive function could be used as valid tools to predict functional outcomes after stroke .
	manualset3
127895	1	405762	13	NULL	NULL	0	NULL	Putative cobreeding males	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Putative cobreeding males within social groups shared paternity .
	manualset3
127896	2	405762	13	NULL	NULL	0	NULL	social groups 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Putative cobreeding males within social groups shared paternity .
	manualset3
128889	3	405762	13	NULL	NULL	0	NULL	paternity	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Putative cobreeding males within social groups shared paternity .
	manualset3
127897	1	405763	13	NULL	NULL	0	NULL	Putative transmitters	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Putative transmitters and related substances were perfused through the guinea pig scala tympani while monitoring the compound action potential of the cochlear nerve ( AP ) and the cochlear microphonic potential .
	manualset3
127898	2	405763	13	NULL	NULL	0	NULL	related substances 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Putative transmitters and related substances were perfused through the guinea pig scala tympani while monitoring the compound action potential of the cochlear nerve ( AP ) and the cochlear microphonic potential .
	manualset3
127899	3	405763	13	NULL	NULL	0	NULL	guinea pig scala tympani	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Putative transmitters and related substances were perfused through the guinea pig scala tympani while monitoring the compound action potential of the cochlear nerve ( AP ) and the cochlear microphonic potential .
	manualset3
127900	4	405763	13	NULL	NULL	0	NULL	compound action potential	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Putative transmitters and related substances were perfused through the guinea pig scala tympani while monitoring the compound action potential of the cochlear nerve ( AP ) and the cochlear microphonic potential .
	manualset3
127901	5	405763	13	NULL	NULL	0	NULL	cochlear nerve ( AP ) 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Putative transmitters and related substances were perfused through the guinea pig scala tympani while monitoring the compound action potential of the cochlear nerve ( AP ) and the cochlear microphonic potential .
	manualset3
127902	6	405763	13	NULL	NULL	0	NULL	cochlear microphonic potential 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Putative transmitters and related substances were perfused through the guinea pig scala tympani while monitoring the compound action potential of the cochlear nerve ( AP ) and the cochlear microphonic potential .
	manualset3
127903	1	405764	13	NULL	NULL	0	NULL	choice 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Putting choice back into the health care equation .
	manualset3
127904	2	405764	13	NULL	NULL	NULL	NULL	health care	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Putting choice back into the health care equation .
	manualset3
128890	3	405764	13	NULL	NULL	0	NULL	equation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Putting choice back into the health care equation .
	manualset3
127905	1	405765	13	NULL	NULL	0	NULL	cuffs 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Putting the cuffs on chest pain .
	manualset3
127906	2	405765	13	NULL	NULL	0	NULL	chest pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Putting the cuffs on chest pain .
	manualset3
127907	1	405766	13	NULL	NULL	0	NULL	Pylephlebitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pylephlebitis is a condition with significant morbidity and mortality .
	manualset3
127908	2	405766	13	NULL	NULL	0	NULL	condition 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pylephlebitis is a condition with significant morbidity and mortality .
	manualset3
127909	3	405766	13	NULL	NULL	0	NULL	morbidity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pylephlebitis is a condition with significant morbidity and mortality .
	manualset3
127910	4	405766	13	NULL	NULL	0	NULL	mortality 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pylephlebitis is a condition with significant morbidity and mortality .
	manualset3
127911	1	405767	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A marked increase in heart rate after drug administration was seen in some patients with AF , which reflects the supersensitivity to denopamine .
	manualset3
127912	2	405767	13	NULL	NULL	0	NULL	heart rate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A marked increase in heart rate after drug administration was seen in some patients with AF , which reflects the supersensitivity to denopamine .
	manualset3
127913	3	405767	13	NULL	NULL	0	NULL	drug administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A marked increase in heart rate after drug administration was seen in some patients with AF , which reflects the supersensitivity to denopamine .
	manualset3
127914	4	405767	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A marked increase in heart rate after drug administration was seen in some patients with AF , which reflects the supersensitivity to denopamine .
	manualset3
127915	5	405767	13	NULL	NULL	0	NULL	AF	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A marked increase in heart rate after drug administration was seen in some patients with AF , which reflects the supersensitivity to denopamine .
	manualset3
127916	6	405767	13	NULL	NULL	0	NULL	supersensitivity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A marked increase in heart rate after drug administration was seen in some patients with AF , which reflects the supersensitivity to denopamine .
	manualset3
127917	7	405767	13	NULL	NULL	0	NULL	denopamine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A marked increase in heart rate after drug administration was seen in some patients with AF , which reflects the supersensitivity to denopamine .
	manualset3
127918	1	405768	13	NULL	NULL	0	NULL	Pyridoxal 5 ' - phosphate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Pyridoxal 5 ' - phosphate also showed a potency to dissociate the 1 , 25 - ( OH ) 2D3-receptor complex previously bound to DNA-cellulose .
	manualset3
127919	2	405768	13	NULL	NULL	0	NULL	potency	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pyridoxal 5 ' - phosphate also showed a potency to dissociate the 1 , 25 - ( OH ) 2D3-receptor complex previously bound to DNA-cellulose .
	manualset3
127920	3	405768	13	NULL	NULL	0	NULL	1 , 25 - ( OH ) 2D3-receptor complex 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Pyridoxal 5 ' - phosphate also showed a potency to dissociate the 1 , 25 - ( OH ) 2D3-receptor complex previously bound to DNA-cellulose .
	manualset3
127921	4	405768	13	NULL	NULL	0	NULL	DNA-cellulose	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Pyridoxal 5 ' - phosphate also showed a potency to dissociate the 1 , 25 - ( OH ) 2D3-receptor complex previously bound to DNA-cellulose .
	manualset3
127922	1	405769	13	NULL	NULL	0	NULL	Pyroglutamic acid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Pyroglutamic acid markedly stimulated brain metabolism : increased glucose uptake and utilization by cerebral tissues and decreased brain lactate dehydrogenase activity .
	manualset3
127923	2	405769	13	NULL	NULL	NULL	NULL	brain metabolism	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pyroglutamic acid markedly stimulated brain metabolism : increased glucose uptake and utilization by cerebral tissues and decreased brain lactate dehydrogenase activity .
	manualset3
127925	4	405769	13	NULL	NULL	0	NULL	glucose uptake	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pyroglutamic acid markedly stimulated brain metabolism : increased glucose uptake and utilization by cerebral tissues and decreased brain lactate dehydrogenase activity .
	manualset3
127926	5	405769	13	NULL	NULL	0	NULL	utilization 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pyroglutamic acid markedly stimulated brain metabolism : increased glucose uptake and utilization by cerebral tissues and decreased brain lactate dehydrogenase activity .
	manualset3
127927	6	405769	13	NULL	NULL	0	NULL	cerebral tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Pyroglutamic acid markedly stimulated brain metabolism : increased glucose uptake and utilization by cerebral tissues and decreased brain lactate dehydrogenase activity .
	manualset3
127928	7	405769	13	NULL	NULL	NULL	NULL	brain lactate dehydrogenase activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pyroglutamic acid markedly stimulated brain metabolism : increased glucose uptake and utilization by cerebral tissues and decreased brain lactate dehydrogenase activity .
	manualset3
127930	1	405770	13	NULL	NULL	0	NULL	Pyrosequencing technology 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pyrosequencing technology , sequencing by addition , was evaluated for categorization of mycobacterial isolates .
	manualset3
127931	2	405770	13	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pyrosequencing technology , sequencing by addition , was evaluated for categorization of mycobacterial isolates .
	manualset3
127932	3	405770	13	NULL	NULL	0	NULL	categorization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pyrosequencing technology , sequencing by addition , was evaluated for categorization of mycobacterial isolates .
	manualset3
127933	4	405770	13	NULL	NULL	0	NULL	mycobacterial isolates 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pyrosequencing technology , sequencing by addition , was evaluated for categorization of mycobacterial isolates .
	manualset3
128891	5	405770	13	NULL	NULL	0	NULL	sequencing 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pyrosequencing technology , sequencing by addition , was evaluated for categorization of mycobacterial isolates .
	manualset3
127934	1	405771	13	NULL	NULL	0	NULL	Q-PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Q-PCR was used to confirm that freshly isolated peripheral blood leukocytes ( PBLs ) express ERs .
	manualset3
127935	2	405771	13	NULL	NULL	0	NULL	 peripheral blood leukocytes ( PBLs )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Q-PCR was used to confirm that freshly isolated peripheral blood leukocytes ( PBLs ) express ERs .
	manualset3
127936	3	405771	13	NULL	NULL	0	NULL	ERs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Q-PCR was used to confirm that freshly isolated peripheral blood leukocytes ( PBLs ) express ERs .
	manualset3
127937	1	405772	13	NULL	NULL	0	NULL	QC	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	QC should be performed frequently enough that QCM are used cost-effectively and that POCA analytical error can be reliably detected .
	manualset3
127938	2	405772	13	NULL	NULL	0	NULL	QCM	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	QC should be performed frequently enough that QCM are used cost-effectively and that POCA analytical error can be reliably detected .
	manualset3
127939	3	405772	13	NULL	NULL	0	NULL	POCA analytical error	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	QC should be performed frequently enough that QCM are used cost-effectively and that POCA analytical error can be reliably detected .
	manualset3
127940	1	405773	13	NULL	NULL	0	NULL	QT dispersion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	QT dispersion and heart rate variability abnormalities in Alzheimer 's disease and in mild cognitive impairment .
	manualset3
127941	2	405773	13	NULL	NULL	0	NULL	heart rate variability abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	QT dispersion and heart rate variability abnormalities in Alzheimer 's disease and in mild cognitive impairment .
	manualset3
127942	3	405773	13	NULL	NULL	0	NULL	Alzheimer 's disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	QT dispersion and heart rate variability abnormalities in Alzheimer 's disease and in mild cognitive impairment .
	manualset3
127943	4	405773	13	NULL	NULL	0	NULL	mild cognitive impairment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	QT dispersion and heart rate variability abnormalities in Alzheimer 's disease and in mild cognitive impairment .
	manualset3
127944	1	405774	13	NULL	NULL	0	NULL	QTL mapping	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	QTL mapping in a mouse model of cardiomyopathy reveals an ancestral modifier allele affecting heart function and survival .
	manualset3
127945	2	405774	13	NULL	NULL	0	NULL	 mouse model of cardiomyopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	QTL mapping in a mouse model of cardiomyopathy reveals an ancestral modifier allele affecting heart function and survival .
	manualset3
127946	3	405774	13	NULL	NULL	0	NULL	modifier allele	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	QTL mapping in a mouse model of cardiomyopathy reveals an ancestral modifier allele affecting heart function and survival .
	manualset3
127947	4	405774	13	NULL	NULL	0	NULL	heart function 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	QTL mapping in a mouse model of cardiomyopathy reveals an ancestral modifier allele affecting heart function and survival .
	manualset3
127948	5	405774	13	NULL	NULL	0	NULL	survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	QTL mapping in a mouse model of cardiomyopathy reveals an ancestral modifier allele affecting heart function and survival .
	manualset3
127949	1	405775	13	NULL	NULL	0	NULL	market basket survey	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A market basket survey of produce conducted between October 1996 and May 1997 in Trinidad for organophosphate pesticides showed that 10 % of produce exceeded the internationally acceptable maximum residue limits ( MRLs ) for the respective pesticides .
	manualset3
127950	2	405775	13	NULL	NULL	NULL	NULL	produce	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A market basket survey of produce conducted between October 1996 and May 1997 in Trinidad for organophosphate pesticides showed that 10 % of produce exceeded the internationally acceptable maximum residue limits ( MRLs ) for the respective pesticides .
	manualset3
127951	3	405775	13	NULL	NULL	0	NULL	October 1996 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	A market basket survey of produce conducted between October 1996 and May 1997 in Trinidad for organophosphate pesticides showed that 10 % of produce exceeded the internationally acceptable maximum residue limits ( MRLs ) for the respective pesticides .
	manualset3
127952	4	405775	13	NULL	NULL	0	NULL	May 1997	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	A market basket survey of produce conducted between October 1996 and May 1997 in Trinidad for organophosphate pesticides showed that 10 % of produce exceeded the internationally acceptable maximum residue limits ( MRLs ) for the respective pesticides .
	manualset3
127953	5	405775	13	NULL	NULL	0	NULL	Trinidad 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A market basket survey of produce conducted between October 1996 and May 1997 in Trinidad for organophosphate pesticides showed that 10 % of produce exceeded the internationally acceptable maximum residue limits ( MRLs ) for the respective pesticides .
	manualset3
127954	6	405775	13	NULL	NULL	0	NULL	organophosphate pesticides 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A market basket survey of produce conducted between October 1996 and May 1997 in Trinidad for organophosphate pesticides showed that 10 % of produce exceeded the internationally acceptable maximum residue limits ( MRLs ) for the respective pesticides .
	manualset3
127955	7	405775	13	NULL	NULL	0	NULL	10 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A market basket survey of produce conducted between October 1996 and May 1997 in Trinidad for organophosphate pesticides showed that 10 % of produce exceeded the internationally acceptable maximum residue limits ( MRLs ) for the respective pesticides .
	manualset3
127956	8	405775	13	NULL	NULL	0	NULL	produce	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A market basket survey of produce conducted between October 1996 and May 1997 in Trinidad for organophosphate pesticides showed that 10 % of produce exceeded the internationally acceptable maximum residue limits ( MRLs ) for the respective pesticides .
	manualset3
127957	9	405775	13	NULL	NULL	0	NULL	maximum residue limits ( MRLs ) 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A market basket survey of produce conducted between October 1996 and May 1997 in Trinidad for organophosphate pesticides showed that 10 % of produce exceeded the internationally acceptable maximum residue limits ( MRLs ) for the respective pesticides .
	manualset3
127958	10	405775	13	NULL	NULL	0	NULL	pesticides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A market basket survey of produce conducted between October 1996 and May 1997 in Trinidad for organophosphate pesticides showed that 10 % of produce exceeded the internationally acceptable maximum residue limits ( MRLs ) for the respective pesticides .
	manualset3
127959	1	405776	13	NULL	NULL	0	NULL	QUIN	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	QUIN ( 10 microM ) antagonized methacholine-stimulated contractile responses in a noncompetitive manner in rings devoid of endothelium .
	manualset3
127960	2	405776	13	NULL	NULL	0	NULL	10 microM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	QUIN ( 10 microM ) antagonized methacholine-stimulated contractile responses in a noncompetitive manner in rings devoid of endothelium .
	manualset3
127961	3	405776	13	NULL	NULL	NULL	NULL	methacholine-stimulated contractile responses 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	QUIN ( 10 microM ) antagonized methacholine-stimulated contractile responses in a noncompetitive manner in rings devoid of endothelium .
	manualset3
127962	4	405776	13	NULL	NULL	0	NULL	noncompetitive manner	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	QUIN ( 10 microM ) antagonized methacholine-stimulated contractile responses in a noncompetitive manner in rings devoid of endothelium .
	manualset3
127963	5	405776	13	NULL	NULL	0	NULL	rings	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	QUIN ( 10 microM ) antagonized methacholine-stimulated contractile responses in a noncompetitive manner in rings devoid of endothelium .
	manualset3
127964	6	405776	13	NULL	NULL	0	NULL	endothelium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	QUIN ( 10 microM ) antagonized methacholine-stimulated contractile responses in a noncompetitive manner in rings devoid of endothelium .
	manualset3
127965	1	405777	13	NULL	NULL	0	NULL	Qualitative analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Qualitative analysis of parent experiences with achieving cystic fibrosis nutrition recommendations .
	manualset3
127966	2	405777	13	NULL	NULL	0	NULL	parent experiences 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Qualitative analysis of parent experiences with achieving cystic fibrosis nutrition recommendations .
	manualset3
127967	3	405777	13	NULL	NULL	0	NULL	cystic fibrosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Qualitative analysis of parent experiences with achieving cystic fibrosis nutrition recommendations .
	manualset3
127968	4	405777	13	NULL	NULL	0	NULL	nutrition recommendations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Qualitative analysis of parent experiences with achieving cystic fibrosis nutrition recommendations .
	manualset3
127969	1	405778	13	NULL	NULL	0	NULL	Qualitative analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Qualitative and quantitative analyses ( author 's transl ) ) .
	manualset3
127970	2	405778	13	NULL	NULL	0	NULL	quantitative analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Qualitative and quantitative analyses ( author 's transl ) ) .
	manualset3
127971	3	405778	13	NULL	NULL	0	NULL	author 's	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Qualitative and quantitative analyses ( author 's transl ) ) .
	manualset3
127972	1	405779	13	NULL	NULL	0	NULL	Qualitative descriptions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Qualitative and quantitative descriptions of temperature : a study of the terminology used by local television weather forecasters to describe thermal sensation .
	manualset3
127973	2	405779	13	NULL	NULL	0	NULL	quantitative descriptions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Qualitative and quantitative descriptions of temperature : a study of the terminology used by local television weather forecasters to describe thermal sensation .
	manualset3
127974	3	405779	13	NULL	NULL	0	NULL	temperature	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Qualitative and quantitative descriptions of temperature : a study of the terminology used by local television weather forecasters to describe thermal sensation .
	manualset3
127975	4	405779	13	NULL	NULL	0	NULL	study	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Qualitative and quantitative descriptions of temperature : a study of the terminology used by local television weather forecasters to describe thermal sensation .
	manualset3
127976	5	405779	13	NULL	NULL	0	NULL	terminology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Qualitative and quantitative descriptions of temperature : a study of the terminology used by local television weather forecasters to describe thermal sensation .
	manualset3
127977	6	405779	13	NULL	NULL	0	NULL	television	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Qualitative and quantitative descriptions of temperature : a study of the terminology used by local television weather forecasters to describe thermal sensation .
	manualset3
127978	7	405779	13	NULL	NULL	0	NULL	weather forecasters	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Qualitative and quantitative descriptions of temperature : a study of the terminology used by local television weather forecasters to describe thermal sensation .
	manualset3
127979	8	405779	13	NULL	NULL	0	NULL	thermal sensation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Qualitative and quantitative descriptions of temperature : a study of the terminology used by local television weather forecasters to describe thermal sensation .
	manualset3
127980	1	405780	13	NULL	NULL	0	NULL	Qualitative studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Qualitative and quantitative studies on mixed homologous chicken thymus cell cultures .
	manualset3
127981	2	405780	13	NULL	NULL	0	NULL	quantitative studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Qualitative and quantitative studies on mixed homologous chicken thymus cell cultures .
	manualset3
127982	3	405780	13	NULL	NULL	0	NULL	homologous chicken thymus cell cultures 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Qualitative and quantitative studies on mixed homologous chicken thymus cell cultures .
	manualset3
127983	1	405781	13	NULL	NULL	0	NULL	mass fragmentographic method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A mass fragmentographic method for the determination of total cholesterol in serum using heptadeuterated ( 25 , 26 , 26 , 26 , 27 , 27 , 27-2H ) cholesterol as internal standard is presented .
	manualset3
127984	2	405781	13	NULL	NULL	0	NULL	determination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A mass fragmentographic method for the determination of total cholesterol in serum using heptadeuterated ( 25 , 26 , 26 , 26 , 27 , 27 , 27-2H ) cholesterol as internal standard is presented .
	manualset3
127985	3	405781	13	NULL	NULL	0	NULL	total cholesterol 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A mass fragmentographic method for the determination of total cholesterol in serum using heptadeuterated ( 25 , 26 , 26 , 26 , 27 , 27 , 27-2H ) cholesterol as internal standard is presented .
	manualset3
127986	4	405781	13	NULL	NULL	0	NULL	serum 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A mass fragmentographic method for the determination of total cholesterol in serum using heptadeuterated ( 25 , 26 , 26 , 26 , 27 , 27 , 27-2H ) cholesterol as internal standard is presented .
	manualset3
127987	5	405781	13	NULL	NULL	0	NULL	heptadeuterated ( 25 , 26 , 26 , 26 , 27 , 27 , 27-2H ) cholesterol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A mass fragmentographic method for the determination of total cholesterol in serum using heptadeuterated ( 25 , 26 , 26 , 26 , 27 , 27 , 27-2H ) cholesterol as internal standard is presented .
	manualset3
127988	6	405781	13	NULL	NULL	0	NULL	standard	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A mass fragmentographic method for the determination of total cholesterol in serum using heptadeuterated ( 25 , 26 , 26 , 26 , 27 , 27 , 27-2H ) cholesterol as internal standard is presented .
	manualset3
127989	1	405782	13	NULL	NULL	0	NULL	Quantal release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantal release of calcium in permeabilized A7r5 cells is not caused by intrinsic inactivation of the inositol trisphosphate receptor .
	manualset3
127990	2	405782	13	NULL	NULL	0	NULL	calcium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantal release of calcium in permeabilized A7r5 cells is not caused by intrinsic inactivation of the inositol trisphosphate receptor .
	manualset3
127991	3	405782	13	NULL	NULL	0	NULL	A7r5 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantal release of calcium in permeabilized A7r5 cells is not caused by intrinsic inactivation of the inositol trisphosphate receptor .
	manualset3
127992	4	405782	13	NULL	NULL	0	NULL	inactivation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantal release of calcium in permeabilized A7r5 cells is not caused by intrinsic inactivation of the inositol trisphosphate receptor .
	manualset3
127993	5	405782	13	NULL	NULL	0	NULL	inositol trisphosphate receptor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantal release of calcium in permeabilized A7r5 cells is not caused by intrinsic inactivation of the inositol trisphosphate receptor .
	manualset3
127994	1	405783	13	NULL	NULL	0	NULL	Quantification 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of HPV-16 E6-E7 transcription in cervical intraepithelial neoplasia by reverse transcriptase polymerase chain reaction .
	manualset3
127995	2	405783	13	NULL	NULL	NULL	NULL	HPV-16 E6-E7 transcription 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Quantification of HPV-16 E6-E7 transcription in cervical intraepithelial neoplasia by reverse transcriptase polymerase chain reaction .
	manualset3
127996	3	405783	13	NULL	NULL	0	NULL	cervical intraepithelial neoplasia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of HPV-16 E6-E7 transcription in cervical intraepithelial neoplasia by reverse transcriptase polymerase chain reaction .
	manualset3
127997	4	405783	13	NULL	NULL	0	NULL	reverse transcriptase polymerase chain reaction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of HPV-16 E6-E7 transcription in cervical intraepithelial neoplasia by reverse transcriptase polymerase chain reaction .
	manualset3
127998	1	405784	13	NULL	NULL	0	NULL	Quantification 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of TNF-alpha and IL-6 mRNA in RAW264 .7 cells by real-time RT-PCR revealed that both sophocarpine and matrine suppressed TNF-alpha and IL-6 expression and sophocarpine has stronger suppressing potency than matrine .
	manualset3
127999	2	405784	13	NULL	NULL	0	NULL	TNF-alpha mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of TNF-alpha and IL-6 mRNA in RAW264 .7 cells by real-time RT-PCR revealed that both sophocarpine and matrine suppressed TNF-alpha and IL-6 expression and sophocarpine has stronger suppressing potency than matrine .
	manualset3
128000	3	405784	13	NULL	NULL	0	NULL	IL-6 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of TNF-alpha and IL-6 mRNA in RAW264 .7 cells by real-time RT-PCR revealed that both sophocarpine and matrine suppressed TNF-alpha and IL-6 expression and sophocarpine has stronger suppressing potency than matrine .
	manualset3
128001	4	405784	13	NULL	NULL	0	NULL	RAW264 .7 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of TNF-alpha and IL-6 mRNA in RAW264 .7 cells by real-time RT-PCR revealed that both sophocarpine and matrine suppressed TNF-alpha and IL-6 expression and sophocarpine has stronger suppressing potency than matrine .
	manualset3
128002	5	405784	13	NULL	NULL	0	NULL	real-time RT-PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of TNF-alpha and IL-6 mRNA in RAW264 .7 cells by real-time RT-PCR revealed that both sophocarpine and matrine suppressed TNF-alpha and IL-6 expression and sophocarpine has stronger suppressing potency than matrine .
	manualset3
128003	6	405784	13	NULL	NULL	0	NULL	sophocarpine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of TNF-alpha and IL-6 mRNA in RAW264 .7 cells by real-time RT-PCR revealed that both sophocarpine and matrine suppressed TNF-alpha and IL-6 expression and sophocarpine has stronger suppressing potency than matrine .
	manualset3
128004	7	405784	13	NULL	NULL	0	NULL	matrine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of TNF-alpha and IL-6 mRNA in RAW264 .7 cells by real-time RT-PCR revealed that both sophocarpine and matrine suppressed TNF-alpha and IL-6 expression and sophocarpine has stronger suppressing potency than matrine .
	manualset3
128005	8	405784	13	NULL	NULL	NULL	NULL	TNF-alpha expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Quantification of TNF-alpha and IL-6 mRNA in RAW264 .7 cells by real-time RT-PCR revealed that both sophocarpine and matrine suppressed TNF-alpha and IL-6 expression and sophocarpine has stronger suppressing potency than matrine .
	manualset3
128006	9	405784	13	NULL	NULL	0	NULL	IL-6 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of TNF-alpha and IL-6 mRNA in RAW264 .7 cells by real-time RT-PCR revealed that both sophocarpine and matrine suppressed TNF-alpha and IL-6 expression and sophocarpine has stronger suppressing potency than matrine .
	manualset3
128007	10	405784	13	NULL	NULL	0	NULL	sophocarpine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of TNF-alpha and IL-6 mRNA in RAW264 .7 cells by real-time RT-PCR revealed that both sophocarpine and matrine suppressed TNF-alpha and IL-6 expression and sophocarpine has stronger suppressing potency than matrine .
	manualset3
128008	11	405784	13	NULL	NULL	0	NULL	potency	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of TNF-alpha and IL-6 mRNA in RAW264 .7 cells by real-time RT-PCR revealed that both sophocarpine and matrine suppressed TNF-alpha and IL-6 expression and sophocarpine has stronger suppressing potency than matrine .
	manualset3
128009	12	405784	13	NULL	NULL	0	NULL	matrine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of TNF-alpha and IL-6 mRNA in RAW264 .7 cells by real-time RT-PCR revealed that both sophocarpine and matrine suppressed TNF-alpha and IL-6 expression and sophocarpine has stronger suppressing potency than matrine .
	manualset3
128010	1	405785	13	NULL	NULL	NULL	NULL	Quantification	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Quantification of aortic lesions and plasma lipid determination showed that compared with their control apoE ( 0 ) counterparts , the apoA-IV/E ( 0 ) mice are protected against atherosclerosis without an increase in HDL cholesterol .
	manualset3
128011	2	405785	13	NULL	NULL	0	NULL	aortic lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of aortic lesions and plasma lipid determination showed that compared with their control apoE ( 0 ) counterparts , the apoA-IV/E ( 0 ) mice are protected against atherosclerosis without an increase in HDL cholesterol .
	manualset3
128012	3	405785	13	NULL	NULL	NULL	NULL	plasma lipid determination	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Quantification of aortic lesions and plasma lipid determination showed that compared with their control apoE ( 0 ) counterparts , the apoA-IV/E ( 0 ) mice are protected against atherosclerosis without an increase in HDL cholesterol .
	manualset3
128013	4	405785	13	NULL	NULL	0	NULL	control apoE ( 0 ) counterparts	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of aortic lesions and plasma lipid determination showed that compared with their control apoE ( 0 ) counterparts , the apoA-IV/E ( 0 ) mice are protected against atherosclerosis without an increase in HDL cholesterol .
	manualset3
128014	5	405785	13	NULL	NULL	0	NULL	apoA-IV/E ( 0 ) mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of aortic lesions and plasma lipid determination showed that compared with their control apoE ( 0 ) counterparts , the apoA-IV/E ( 0 ) mice are protected against atherosclerosis without an increase in HDL cholesterol .
	manualset3
128015	6	405785	13	NULL	NULL	0	NULL	atherosclerosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of aortic lesions and plasma lipid determination showed that compared with their control apoE ( 0 ) counterparts , the apoA-IV/E ( 0 ) mice are protected against atherosclerosis without an increase in HDL cholesterol .
	manualset3
128016	7	405785	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of aortic lesions and plasma lipid determination showed that compared with their control apoE ( 0 ) counterparts , the apoA-IV/E ( 0 ) mice are protected against atherosclerosis without an increase in HDL cholesterol .
	manualset3
128017	8	405785	13	NULL	NULL	0	NULL	HDL cholesterol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of aortic lesions and plasma lipid determination showed that compared with their control apoE ( 0 ) counterparts , the apoA-IV/E ( 0 ) mice are protected against atherosclerosis without an increase in HDL cholesterol .
	manualset3
128018	1	405786	13	NULL	NULL	0	NULL	Quantification	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of glucose transport and phosphorylation in human skeletal muscle using FDG PET .
	manualset3
128019	2	405786	13	NULL	NULL	0	NULL	glucose transport 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of glucose transport and phosphorylation in human skeletal muscle using FDG PET .
	manualset3
128020	3	405786	13	NULL	NULL	0	NULL	phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of glucose transport and phosphorylation in human skeletal muscle using FDG PET .
	manualset3
128021	4	405786	13	NULL	NULL	0	NULL	human skeletal muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of glucose transport and phosphorylation in human skeletal muscle using FDG PET .
	manualset3
128022	5	405786	13	NULL	NULL	0	NULL	FDG PET 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of glucose transport and phosphorylation in human skeletal muscle using FDG PET .
	manualset3
128023	1	405787	13	NULL	NULL	NULL	NULL	Quantification 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Quantification of second cancer risk is important in terms of patient management , enabling clinicians to make informed decisions with regard to optimal treatment of the initial cancer , balancing efficacy against acute and chronic sequelae .
	manualset3
128024	2	405787	13	NULL	NULL	0	NULL	second cancer risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of second cancer risk is important in terms of patient management , enabling clinicians to make informed decisions with regard to optimal treatment of the initial cancer , balancing efficacy against acute and chronic sequelae .
	manualset3
128025	3	405787	13	NULL	NULL	0	NULL	patient management 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of second cancer risk is important in terms of patient management , enabling clinicians to make informed decisions with regard to optimal treatment of the initial cancer , balancing efficacy against acute and chronic sequelae .
	manualset3
128026	4	405787	13	NULL	NULL	0	NULL	clinicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of second cancer risk is important in terms of patient management , enabling clinicians to make informed decisions with regard to optimal treatment of the initial cancer , balancing efficacy against acute and chronic sequelae .
	manualset3
128027	5	405787	13	NULL	NULL	0	NULL	decisions	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of second cancer risk is important in terms of patient management , enabling clinicians to make informed decisions with regard to optimal treatment of the initial cancer , balancing efficacy against acute and chronic sequelae .
	manualset3
128028	6	405787	13	NULL	NULL	0	NULL	optimal treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of second cancer risk is important in terms of patient management , enabling clinicians to make informed decisions with regard to optimal treatment of the initial cancer , balancing efficacy against acute and chronic sequelae .
	manualset3
128029	7	405787	13	NULL	NULL	0	NULL	cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of second cancer risk is important in terms of patient management , enabling clinicians to make informed decisions with regard to optimal treatment of the initial cancer , balancing efficacy against acute and chronic sequelae .
	manualset3
128030	8	405787	13	NULL	NULL	0	NULL	balancing efficacy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of second cancer risk is important in terms of patient management , enabling clinicians to make informed decisions with regard to optimal treatment of the initial cancer , balancing efficacy against acute and chronic sequelae .
	manualset3
128031	9	405787	13	NULL	NULL	NULL	NULL	acute sequelae 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Quantification of second cancer risk is important in terms of patient management , enabling clinicians to make informed decisions with regard to optimal treatment of the initial cancer , balancing efficacy against acute and chronic sequelae .
	manualset3
128892	10	405787	13	NULL	NULL	0	NULL	chronic sequelae 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of second cancer risk is important in terms of patient management , enabling clinicians to make informed decisions with regard to optimal treatment of the initial cancer , balancing efficacy against acute and chronic sequelae .
	manualset3
128032	1	405788	13	NULL	NULL	0	NULL	Quantification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of volatile compounds in Chinese soy sauce aroma type liquor by stir bar sorptive extraction and gas chromatography-mass spectrometry .
	manualset3
128033	2	405788	13	NULL	NULL	0	NULL	volatile compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of volatile compounds in Chinese soy sauce aroma type liquor by stir bar sorptive extraction and gas chromatography-mass spectrometry .
	manualset3
128034	3	405788	13	NULL	NULL	0	NULL	Chinese soy sauce aroma type liquor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of volatile compounds in Chinese soy sauce aroma type liquor by stir bar sorptive extraction and gas chromatography-mass spectrometry .
	manualset3
128035	4	405788	13	NULL	NULL	0	NULL	stir bar sorptive extraction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of volatile compounds in Chinese soy sauce aroma type liquor by stir bar sorptive extraction and gas chromatography-mass spectrometry .
	manualset3
128036	5	405788	13	NULL	NULL	0	NULL	gas chromatography-mass spectrometry 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantification of volatile compounds in Chinese soy sauce aroma type liquor by stir bar sorptive extraction and gas chromatography-mass spectrometry .
	manualset3
128037	1	405789	13	NULL	NULL	0	NULL	Quantitation analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitation and qualitative analysis of additional photoproducts of RB was also performed , but the method has not been validated for these other components .
	manualset3
128038	2	405789	13	NULL	NULL	0	NULL	qualitative analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitation and qualitative analysis of additional photoproducts of RB was also performed , but the method has not been validated for these other components .
	manualset3
128039	3	405789	13	NULL	NULL	0	NULL	photoproducts of RB	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitation and qualitative analysis of additional photoproducts of RB was also performed , but the method has not been validated for these other components .
	manualset3
128040	4	405789	13	NULL	NULL	0	NULL	method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitation and qualitative analysis of additional photoproducts of RB was also performed , but the method has not been validated for these other components .
	manualset3
128041	5	405789	13	NULL	NULL	0	NULL	components	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitation and qualitative analysis of additional photoproducts of RB was also performed , but the method has not been validated for these other components .
	manualset3
128042	1	405790	13	NULL	NULL	0	NULL	Quantitation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitation of Pyrrole-Imidazole Polyamide in Rat Plasma by High-Performance Liquid Chromatography Coupled with UV Detection .
	manualset3
128043	2	405790	13	NULL	NULL	0	NULL	Pyrrole-Imidazole Polyamide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitation of Pyrrole-Imidazole Polyamide in Rat Plasma by High-Performance Liquid Chromatography Coupled with UV Detection .
	manualset3
128044	3	405790	13	NULL	NULL	0	NULL	Rat Plasma	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitation of Pyrrole-Imidazole Polyamide in Rat Plasma by High-Performance Liquid Chromatography Coupled with UV Detection .
	manualset3
128045	4	405790	13	NULL	NULL	0	NULL	High-Performance Liquid Chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitation of Pyrrole-Imidazole Polyamide in Rat Plasma by High-Performance Liquid Chromatography Coupled with UV Detection .
	manualset3
128046	5	405790	13	NULL	NULL	0	NULL	UV Detection 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitation of Pyrrole-Imidazole Polyamide in Rat Plasma by High-Performance Liquid Chromatography Coupled with UV Detection .
	manualset3
128047	1	405791	13	NULL	NULL	0	NULL	Quantitation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitation of soluble HLA-DR antigens in human serum and other body fluids .
	manualset3
128048	2	405791	13	NULL	NULL	0	NULL	soluble HLA-DR antigens	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitation of soluble HLA-DR antigens in human serum and other body fluids .
	manualset3
128049	3	405791	13	NULL	NULL	NULL	NULL	 human serum 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Quantitation of soluble HLA-DR antigens in human serum and other body fluids .
	manualset3
128050	4	405791	13	NULL	NULL	NULL	NULL	body fluids	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Quantitation of soluble HLA-DR antigens in human serum and other body fluids .
	manualset3
128051	1	405792	13	NULL	NULL	0	NULL	Quantitative 45 Ca autoradiography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative 45 Ca autoradiography of human bone .
	manualset3
128052	2	405792	13	NULL	NULL	0	NULL	human bone	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative 45 Ca autoradiography of human bone .
	manualset3
128053	1	405793	13	NULL	NULL	0	NULL	Quantitative PCR ( qPCR ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative PCR ( qPCR ) is a method for rapid and reliable quantification of mRNA .
	manualset3
128054	2	405793	13	NULL	NULL	0	NULL	method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative PCR ( qPCR ) is a method for rapid and reliable quantification of mRNA .
	manualset3
128055	3	405793	13	NULL	NULL	0	NULL	quantification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative PCR ( qPCR ) is a method for rapid and reliable quantification of mRNA .
	manualset3
128056	4	405793	13	NULL	NULL	0	NULL	mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative PCR ( qPCR ) is a method for rapid and reliable quantification of mRNA .
	manualset3
128057	1	405794	13	NULL	NULL	0	NULL	Quantitative PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative PCR to evaluate small amounts of BCL2 mRNA in human peripheral T cells : implication of equimolar target and competitor end products .
	manualset3
128058	2	405794	13	NULL	NULL	0	NULL	amounts	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative PCR to evaluate small amounts of BCL2 mRNA in human peripheral T cells : implication of equimolar target and competitor end products .
	manualset3
128059	3	405794	13	NULL	NULL	0	NULL	BCL2 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative PCR to evaluate small amounts of BCL2 mRNA in human peripheral T cells : implication of equimolar target and competitor end products .
	manualset3
128060	4	405794	13	NULL	NULL	0	NULL	human peripheral T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative PCR to evaluate small amounts of BCL2 mRNA in human peripheral T cells : implication of equimolar target and competitor end products .
	manualset3
128061	5	405794	13	NULL	NULL	0	NULL	implication	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative PCR to evaluate small amounts of BCL2 mRNA in human peripheral T cells : implication of equimolar target and competitor end products .
	manualset3
128062	6	405794	13	NULL	NULL	0	NULL	equimolar target	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative PCR to evaluate small amounts of BCL2 mRNA in human peripheral T cells : implication of equimolar target and competitor end products .
	manualset3
128063	7	405794	13	NULL	NULL	0	NULL	competitor end products	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative PCR to evaluate small amounts of BCL2 mRNA in human peripheral T cells : implication of equimolar target and competitor end products .
	manualset3
128064	1	405795	13	NULL	NULL	0	NULL	Quantitative analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative analysis of ascaridol , a heat-sensitive compound , was carried out by 13C NMR spectroscopy .
	manualset3
128065	2	405795	13	NULL	NULL	0	NULL	ascaridol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative analysis of ascaridol , a heat-sensitive compound , was carried out by 13C NMR spectroscopy .
	manualset3
128066	3	405795	13	NULL	NULL	0	NULL	heat-sensitive compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative analysis of ascaridol , a heat-sensitive compound , was carried out by 13C NMR spectroscopy .
	manualset3
128067	4	405795	13	NULL	NULL	0	NULL	13C NMR spectroscopy 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative analysis of ascaridol , a heat-sensitive compound , was carried out by 13C NMR spectroscopy .
	manualset3
128068	1	405796	13	NULL	NULL	NULL	NULL	Quantitative analysis	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Quantitative analysis of glycogen content in hepatocytes of human liver allograft after ischemia and reperfusion .
	manualset3
128069	2	405796	13	NULL	NULL	0	NULL	glycogen content 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative analysis of glycogen content in hepatocytes of human liver allograft after ischemia and reperfusion .
	manualset3
128071	3	405796	13	NULL	NULL	0	NULL	hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative analysis of glycogen content in hepatocytes of human liver allograft after ischemia and reperfusion .
	manualset3
128072	4	405796	13	NULL	NULL	0	NULL	human liver allograft	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative analysis of glycogen content in hepatocytes of human liver allograft after ischemia and reperfusion .
	manualset3
128073	5	405796	13	NULL	NULL	0	NULL	ischemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative analysis of glycogen content in hepatocytes of human liver allograft after ischemia and reperfusion .
	manualset3
128074	6	405796	13	NULL	NULL	0	NULL	reperfusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative analysis of glycogen content in hepatocytes of human liver allograft after ischemia and reperfusion .
	manualset3
128075	1	405797	13	NULL	NULL	NULL	NULL	Quantitative analysis	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Quantitative analysis of liposuction with B mode ultrasound .
	manualset3
128076	2	405797	13	NULL	NULL	0	NULL	liposuction	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative analysis of liposuction with B mode ultrasound .
	manualset3
128077	3	405797	13	NULL	NULL	0	NULL	B mode ultrasound	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative analysis of liposuction with B mode ultrasound .
	manualset3
128078	1	405798	13	NULL	NULL	0	NULL	Quantitative analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative analysis of striatal binding ratios failed to depict these different degeneration patterns in PD and APS patients .
	manualset3
128079	2	405798	13	NULL	NULL	0	NULL	striatal binding ratios 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative analysis of striatal binding ratios failed to depict these different degeneration patterns in PD and APS patients .
	manualset3
128080	3	405798	13	NULL	NULL	0	NULL	degeneration patterns 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative analysis of striatal binding ratios failed to depict these different degeneration patterns in PD and APS patients .
	manualset3
128081	4	405798	13	NULL	NULL	0	NULL	PD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative analysis of striatal binding ratios failed to depict these different degeneration patterns in PD and APS patients .
	manualset3
128082	5	405798	13	NULL	NULL	0	NULL	APS patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative analysis of striatal binding ratios failed to depict these different degeneration patterns in PD and APS patients .
	manualset3
128083	1	405799	13	NULL	NULL	0	NULL	Quantitative aspects 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative aspects of data would indicate that this is due to minute amounts of complementary viral RNA associated with the virion or with the virion RNA itself .
	manualset3
128084	2	405799	13	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative aspects of data would indicate that this is due to minute amounts of complementary viral RNA associated with the virion or with the virion RNA itself .
	manualset3
128085	3	405799	13	NULL	NULL	0	NULL	minute amounts	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative aspects of data would indicate that this is due to minute amounts of complementary viral RNA associated with the virion or with the virion RNA itself .
	manualset3
128086	4	405799	13	NULL	NULL	0	NULL	complementary viral RNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative aspects of data would indicate that this is due to minute amounts of complementary viral RNA associated with the virion or with the virion RNA itself .
	manualset3
128087	5	405799	13	NULL	NULL	0	NULL	virion	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative aspects of data would indicate that this is due to minute amounts of complementary viral RNA associated with the virion or with the virion RNA itself .
	manualset3
128088	6	405799	13	NULL	NULL	0	NULL	virion RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative aspects of data would indicate that this is due to minute amounts of complementary viral RNA associated with the virion or with the virion RNA itself .
	manualset3
128089	1	405800	13	NULL	NULL	0	NULL	Quantitative assessment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative assessment of LMP2 , MECL1 , and LMP7 transcripts revealed that the inhibition of immunoproteasome formation occurred at a pretranscriptional level .
	manualset3
128090	2	405800	13	NULL	NULL	0	NULL	LMP2 transcript	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative assessment of LMP2 , MECL1 , and LMP7 transcripts revealed that the inhibition of immunoproteasome formation occurred at a pretranscriptional level .
	manualset3
128091	3	405800	13	NULL	NULL	0	NULL	MECL1 transcript	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative assessment of LMP2 , MECL1 , and LMP7 transcripts revealed that the inhibition of immunoproteasome formation occurred at a pretranscriptional level .
	manualset3
128092	4	405800	13	NULL	NULL	0	NULL	LMP7 transcript	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative assessment of LMP2 , MECL1 , and LMP7 transcripts revealed that the inhibition of immunoproteasome formation occurred at a pretranscriptional level .
	manualset3
128093	5	405800	13	NULL	NULL	0	NULL	inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative assessment of LMP2 , MECL1 , and LMP7 transcripts revealed that the inhibition of immunoproteasome formation occurred at a pretranscriptional level .
	manualset3
128094	6	405800	13	NULL	NULL	0	NULL	immunoproteasome formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative assessment of LMP2 , MECL1 , and LMP7 transcripts revealed that the inhibition of immunoproteasome formation occurred at a pretranscriptional level .
	manualset3
128095	7	405800	13	NULL	NULL	0	NULL	pretranscriptional level 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative assessment of LMP2 , MECL1 , and LMP7 transcripts revealed that the inhibition of immunoproteasome formation occurred at a pretranscriptional level .
	manualset3
128096	1	405801	13	NULL	NULL	0	NULL	Quantitative binding experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative binding experiments show that nanomolar concentrations of the doubly phosphorylated zeta 1-ITAM are sufficient for ZAP-70 recruitment , whereas micromolar levels of singly phosphorylated ITAM are necessary for p59fyn binding .
	manualset3
128097	2	405801	13	NULL	NULL	0	NULL	nanomolar concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative binding experiments show that nanomolar concentrations of the doubly phosphorylated zeta 1-ITAM are sufficient for ZAP-70 recruitment , whereas micromolar levels of singly phosphorylated ITAM are necessary for p59fyn binding .
	manualset3
128098	3	405801	13	NULL	NULL	NULL	NULL	phosphorylated zeta 1-ITAM	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Quantitative binding experiments show that nanomolar concentrations of the doubly phosphorylated zeta 1-ITAM are sufficient for ZAP-70 recruitment , whereas micromolar levels of singly phosphorylated ITAM are necessary for p59fyn binding .
	manualset3
128099	4	405801	13	NULL	NULL	0	NULL	ZAP-70 recruitment	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative binding experiments show that nanomolar concentrations of the doubly phosphorylated zeta 1-ITAM are sufficient for ZAP-70 recruitment , whereas micromolar levels of singly phosphorylated ITAM are necessary for p59fyn binding .
	manualset3
128100	5	405801	13	NULL	NULL	0	NULL	micromolar levels 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative binding experiments show that nanomolar concentrations of the doubly phosphorylated zeta 1-ITAM are sufficient for ZAP-70 recruitment , whereas micromolar levels of singly phosphorylated ITAM are necessary for p59fyn binding .
	manualset3
128101	6	405801	13	NULL	NULL	NULL	NULL	phosphorylated ITAM	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Quantitative binding experiments show that nanomolar concentrations of the doubly phosphorylated zeta 1-ITAM are sufficient for ZAP-70 recruitment , whereas micromolar levels of singly phosphorylated ITAM are necessary for p59fyn binding .
	manualset3
128102	7	405801	13	NULL	NULL	0	NULL	p59fyn binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative binding experiments show that nanomolar concentrations of the doubly phosphorylated zeta 1-ITAM are sufficient for ZAP-70 recruitment , whereas micromolar levels of singly phosphorylated ITAM are necessary for p59fyn binding .
	manualset3
128103	1	405802	13	NULL	NULL	0	NULL	Quantitative coronary angiography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative coronary angiography was initially proposed as a method of choice to assess coronary disease progression .
	manualset3
128104	2	405802	13	NULL	NULL	0	NULL	method 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative coronary angiography was initially proposed as a method of choice to assess coronary disease progression .
	manualset3
128105	3	405802	13	NULL	NULL	0	NULL	choice 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative coronary angiography was initially proposed as a method of choice to assess coronary disease progression .
	manualset3
128106	4	405802	13	NULL	NULL	0	NULL	coronary disease progression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative coronary angiography was initially proposed as a method of choice to assess coronary disease progression .
	manualset3
128107	1	405803	13	NULL	NULL	0	NULL	Quantitative cytolytic assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative cytolytic assays demonstrated that the maximum rate of cytolysis by pulmonary lymphocytes obtained from mice immunized intraperitoneally exceeded by 10 - to 20-fold the rate of cytolysis by pulmonary lymphocytes obtained from mice receiving intrapulmonary immunization .
	manualset3
128108	2	405803	13	NULL	NULL	0	NULL	rate of cytolysis	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative cytolytic assays demonstrated that the maximum rate of cytolysis by pulmonary lymphocytes obtained from mice immunized intraperitoneally exceeded by 10 - to 20-fold the rate of cytolysis by pulmonary lymphocytes obtained from mice receiving intrapulmonary immunization .
	manualset3
128109	3	405803	13	NULL	NULL	0	NULL	pulmonary lymphocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative cytolytic assays demonstrated that the maximum rate of cytolysis by pulmonary lymphocytes obtained from mice immunized intraperitoneally exceeded by 10 - to 20-fold the rate of cytolysis by pulmonary lymphocytes obtained from mice receiving intrapulmonary immunization .
	manualset3
128110	4	405803	13	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative cytolytic assays demonstrated that the maximum rate of cytolysis by pulmonary lymphocytes obtained from mice immunized intraperitoneally exceeded by 10 - to 20-fold the rate of cytolysis by pulmonary lymphocytes obtained from mice receiving intrapulmonary immunization .
	manualset3
128111	5	405803	13	NULL	NULL	0	NULL	10 - to 20-fold	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative cytolytic assays demonstrated that the maximum rate of cytolysis by pulmonary lymphocytes obtained from mice immunized intraperitoneally exceeded by 10 - to 20-fold the rate of cytolysis by pulmonary lymphocytes obtained from mice receiving intrapulmonary immunization .
	manualset3
128112	6	405803	13	NULL	NULL	0	NULL	rate of cytolysis	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative cytolytic assays demonstrated that the maximum rate of cytolysis by pulmonary lymphocytes obtained from mice immunized intraperitoneally exceeded by 10 - to 20-fold the rate of cytolysis by pulmonary lymphocytes obtained from mice receiving intrapulmonary immunization .
	manualset3
128113	7	405803	13	NULL	NULL	0	NULL	pulmonary lymphocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative cytolytic assays demonstrated that the maximum rate of cytolysis by pulmonary lymphocytes obtained from mice immunized intraperitoneally exceeded by 10 - to 20-fold the rate of cytolysis by pulmonary lymphocytes obtained from mice receiving intrapulmonary immunization .
	manualset3
128114	8	405803	13	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative cytolytic assays demonstrated that the maximum rate of cytolysis by pulmonary lymphocytes obtained from mice immunized intraperitoneally exceeded by 10 - to 20-fold the rate of cytolysis by pulmonary lymphocytes obtained from mice receiving intrapulmonary immunization .
	manualset3
128115	9	405803	13	NULL	NULL	0	NULL	intrapulmonary immunization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative cytolytic assays demonstrated that the maximum rate of cytolysis by pulmonary lymphocytes obtained from mice immunized intraperitoneally exceeded by 10 - to 20-fold the rate of cytolysis by pulmonary lymphocytes obtained from mice receiving intrapulmonary immunization .
	manualset3
128116	1	405804	13	NULL	NULL	0	NULL	Quantitative determination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative determination of single serum proteins during acute hepatitis in childhood .
	manualset3
128117	2	405804	13	NULL	NULL	0	NULL	single serum proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative determination of single serum proteins during acute hepatitis in childhood .
	manualset3
128118	3	405804	13	NULL	NULL	0	NULL	acute hepatitis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative determination of single serum proteins during acute hepatitis in childhood .
	manualset3
128119	4	405804	13	NULL	NULL	0	NULL	childhood	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative determination of single serum proteins during acute hepatitis in childhood .
	manualset3
128120	1	405805	13	NULL	NULL	0	NULL	Quantitative electro-oculographic recording techniques 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative electro-oculographic recording techniques were used to analyze four characteristic eye movement abnormalities in 21 patients with internuclear ophthalmoplegia ( INO ) .
	manualset3
128121	2	405805	13	NULL	NULL	0	NULL	characteristic eye movement abnormalities 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative electro-oculographic recording techniques were used to analyze four characteristic eye movement abnormalities in 21 patients with internuclear ophthalmoplegia ( INO ) .
	manualset3
128122	3	405805	13	NULL	NULL	0	NULL	four	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative electro-oculographic recording techniques were used to analyze four characteristic eye movement abnormalities in 21 patients with internuclear ophthalmoplegia ( INO ) .
	manualset3
128123	4	405805	13	NULL	NULL	0	NULL	21 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative electro-oculographic recording techniques were used to analyze four characteristic eye movement abnormalities in 21 patients with internuclear ophthalmoplegia ( INO ) .
	manualset3
128124	5	405805	13	NULL	NULL	0	NULL	 internuclear ophthalmoplegia ( INO ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative electro-oculographic recording techniques were used to analyze four characteristic eye movement abnormalities in 21 patients with internuclear ophthalmoplegia ( INO ) .
	manualset3
128125	1	405806	13	NULL	NULL	0	NULL	Quantitative evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative evaluation , statistical analyses and MALDI-TOF MS characterization of the resolved spots in treated and untreated samples enabled us to identify 38 proteins whose levels were altered in response to salt stress .
	manualset3
128126	2	405806	13	NULL	NULL	0	NULL	statistical analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative evaluation , statistical analyses and MALDI-TOF MS characterization of the resolved spots in treated and untreated samples enabled us to identify 38 proteins whose levels were altered in response to salt stress .
	manualset3
128127	3	405806	13	NULL	NULL	0	NULL	MALDI-TOF MS characterization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative evaluation , statistical analyses and MALDI-TOF MS characterization of the resolved spots in treated and untreated samples enabled us to identify 38 proteins whose levels were altered in response to salt stress .
	manualset3
128128	4	405806	13	NULL	NULL	0	NULL	spots 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative evaluation , statistical analyses and MALDI-TOF MS characterization of the resolved spots in treated and untreated samples enabled us to identify 38 proteins whose levels were altered in response to salt stress .
	manualset3
128129	5	405806	13	NULL	NULL	0	NULL	samples 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative evaluation , statistical analyses and MALDI-TOF MS characterization of the resolved spots in treated and untreated samples enabled us to identify 38 proteins whose levels were altered in response to salt stress .
	manualset3
128130	6	405806	13	NULL	NULL	0	NULL	38 proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative evaluation , statistical analyses and MALDI-TOF MS characterization of the resolved spots in treated and untreated samples enabled us to identify 38 proteins whose levels were altered in response to salt stress .
	manualset3
128131	7	405806	13	NULL	NULL	0	NULL	levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative evaluation , statistical analyses and MALDI-TOF MS characterization of the resolved spots in treated and untreated samples enabled us to identify 38 proteins whose levels were altered in response to salt stress .
	manualset3
128132	8	405806	13	NULL	NULL	NULL	NULL	response	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Quantitative evaluation , statistical analyses and MALDI-TOF MS characterization of the resolved spots in treated and untreated samples enabled us to identify 38 proteins whose levels were altered in response to salt stress .
	manualset3
128133	9	405806	13	NULL	NULL	0	NULL	salt stress	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative evaluation , statistical analyses and MALDI-TOF MS characterization of the resolved spots in treated and untreated samples enabled us to identify 38 proteins whose levels were altered in response to salt stress .
	manualset3
128134	1	405807	13	NULL	NULL	0	NULL	Quantitative muscle hardness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative muscle hardness as a noninvasive means for detecting patients at risk of compartment syndromes .
	manualset3
128135	2	405807	13	NULL	NULL	0	NULL	noninvasive means	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative muscle hardness as a noninvasive means for detecting patients at risk of compartment syndromes .
	manualset3
128136	3	405807	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative muscle hardness as a noninvasive means for detecting patients at risk of compartment syndromes .
	manualset3
128137	4	405807	13	NULL	NULL	0	NULL	risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative muscle hardness as a noninvasive means for detecting patients at risk of compartment syndromes .
	manualset3
128138	5	405807	13	NULL	NULL	0	NULL	compartment syndromes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative muscle hardness as a noninvasive means for detecting patients at risk of compartment syndromes .
	manualset3
128139	1	405808	13	NULL	NULL	0	NULL	Quantitative proteomics 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative proteomics using stable isotope labeling with amino acids in cell culture reveals changes in the cytoplasmic , nuclear , and nucleolar proteomes in Vero cells infected with the coronavirus infectious bronchitis virus .
	manualset3
128140	2	405808	13	NULL	NULL	0	NULL	stable isotope labeling with amino acids in cell culture	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative proteomics using stable isotope labeling with amino acids in cell culture reveals changes in the cytoplasmic , nuclear , and nucleolar proteomes in Vero cells infected with the coronavirus infectious bronchitis virus .
	manualset3
128141	3	405808	13	NULL	NULL	0	NULL	changes 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative proteomics using stable isotope labeling with amino acids in cell culture reveals changes in the cytoplasmic , nuclear , and nucleolar proteomes in Vero cells infected with the coronavirus infectious bronchitis virus .
	manualset3
128142	4	405808	13	NULL	NULL	0	NULL	cytoplasmic proteomes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative proteomics using stable isotope labeling with amino acids in cell culture reveals changes in the cytoplasmic , nuclear , and nucleolar proteomes in Vero cells infected with the coronavirus infectious bronchitis virus .
	manualset3
128143	5	405808	13	NULL	NULL	0	NULL	nuclear proteomes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative proteomics using stable isotope labeling with amino acids in cell culture reveals changes in the cytoplasmic , nuclear , and nucleolar proteomes in Vero cells infected with the coronavirus infectious bronchitis virus .
	manualset3
128144	6	405808	13	NULL	NULL	0	NULL	nucleolar proteomes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative proteomics using stable isotope labeling with amino acids in cell culture reveals changes in the cytoplasmic , nuclear , and nucleolar proteomes in Vero cells infected with the coronavirus infectious bronchitis virus .
	manualset3
128145	7	405808	13	NULL	NULL	0	NULL	Vero cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative proteomics using stable isotope labeling with amino acids in cell culture reveals changes in the cytoplasmic , nuclear , and nucleolar proteomes in Vero cells infected with the coronavirus infectious bronchitis virus .
	manualset3
128146	8	405808	13	NULL	NULL	0	NULL	coronavirus infectious bronchitis virus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative proteomics using stable isotope labeling with amino acids in cell culture reveals changes in the cytoplasmic , nuclear , and nucleolar proteomes in Vero cells infected with the coronavirus infectious bronchitis virus .
	manualset3
128147	1	405809	13	NULL	NULL	0	NULL	Quantitative reverse transcription-polymerase chain reaction ( RT-PCR ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative reverse transcription-polymerase chain reaction ( RT-PCR ) results indicate that approximately 12 h are required for transcription of 1 , 770 kb ( at an average elongation rate of 2.4 kb min-1 ) , extrapolating to a transcription time of 16 h for the complete gene .
	manualset3
128148	2	405809	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative reverse transcription-polymerase chain reaction ( RT-PCR ) results indicate that approximately 12 h are required for transcription of 1 , 770 kb ( at an average elongation rate of 2.4 kb min-1 ) , extrapolating to a transcription time of 16 h for the complete gene .
	manualset3
128149	3	405809	13	NULL	NULL	0	NULL	12 h 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative reverse transcription-polymerase chain reaction ( RT-PCR ) results indicate that approximately 12 h are required for transcription of 1 , 770 kb ( at an average elongation rate of 2.4 kb min-1 ) , extrapolating to a transcription time of 16 h for the complete gene .
	manualset3
128150	4	405809	13	NULL	NULL	0	NULL	transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative reverse transcription-polymerase chain reaction ( RT-PCR ) results indicate that approximately 12 h are required for transcription of 1 , 770 kb ( at an average elongation rate of 2.4 kb min-1 ) , extrapolating to a transcription time of 16 h for the complete gene .
	manualset3
128151	5	405809	13	NULL	NULL	0	NULL	1 , 770 kb	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative reverse transcription-polymerase chain reaction ( RT-PCR ) results indicate that approximately 12 h are required for transcription of 1 , 770 kb ( at an average elongation rate of 2.4 kb min-1 ) , extrapolating to a transcription time of 16 h for the complete gene .
	manualset3
128152	6	405809	13	NULL	NULL	0	NULL	average elongation rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative reverse transcription-polymerase chain reaction ( RT-PCR ) results indicate that approximately 12 h are required for transcription of 1 , 770 kb ( at an average elongation rate of 2.4 kb min-1 ) , extrapolating to a transcription time of 16 h for the complete gene .
	manualset3
128153	7	405809	13	NULL	NULL	0	NULL	2.4 kb min-1 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative reverse transcription-polymerase chain reaction ( RT-PCR ) results indicate that approximately 12 h are required for transcription of 1 , 770 kb ( at an average elongation rate of 2.4 kb min-1 ) , extrapolating to a transcription time of 16 h for the complete gene .
	manualset3
128154	8	405809	13	NULL	NULL	0	NULL	transcription time	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative reverse transcription-polymerase chain reaction ( RT-PCR ) results indicate that approximately 12 h are required for transcription of 1 , 770 kb ( at an average elongation rate of 2.4 kb min-1 ) , extrapolating to a transcription time of 16 h for the complete gene .
	manualset3
128155	9	405809	13	NULL	NULL	0	NULL	16 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative reverse transcription-polymerase chain reaction ( RT-PCR ) results indicate that approximately 12 h are required for transcription of 1 , 770 kb ( at an average elongation rate of 2.4 kb min-1 ) , extrapolating to a transcription time of 16 h for the complete gene .
	manualset3
128156	10	405809	13	NULL	NULL	0	NULL	gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative reverse transcription-polymerase chain reaction ( RT-PCR ) results indicate that approximately 12 h are required for transcription of 1 , 770 kb ( at an average elongation rate of 2.4 kb min-1 ) , extrapolating to a transcription time of 16 h for the complete gene .
	manualset3
128157	1	405810	13	NULL	NULL	0	NULL	mechanism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A mechanism for the effects of decanol on product formation is proposed .
	manualset3
128158	2	405810	13	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A mechanism for the effects of decanol on product formation is proposed .
	manualset3
128159	3	405810	13	NULL	NULL	0	NULL	decanol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A mechanism for the effects of decanol on product formation is proposed .
	manualset3
128160	4	405810	13	NULL	NULL	0	NULL	product 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A mechanism for the effects of decanol on product formation is proposed .
	manualset3
128161	5	405810	13	NULL	NULL	0	NULL	formation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A mechanism for the effects of decanol on product formation is proposed .
	manualset3
128162	1	405811	13	NULL	NULL	0	NULL	Quantitative scanning transmission EM	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative scanning transmission EM of individual collagen fibrils showed abrupt increases and decreases in mass along their axes .
	manualset3
128163	2	405811	13	NULL	NULL	0	NULL	collagen fibrils	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative scanning transmission EM of individual collagen fibrils showed abrupt increases and decreases in mass along their axes .
	manualset3
128166	5	405811	13	NULL	NULL	0	NULL	mass	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative scanning transmission EM of individual collagen fibrils showed abrupt increases and decreases in mass along their axes .
	manualset3
128167	6	405811	13	NULL	NULL	0	NULL	axes 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative scanning transmission EM of individual collagen fibrils showed abrupt increases and decreases in mass along their axes .
	manualset3
128168	1	405812	13	NULL	NULL	0	NULL	Quantitative sputum cell counts 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative sputum cell counts from patients with asthma and chronic bronchitis were performed and found to be reproducible .
	manualset3
128169	2	405812	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative sputum cell counts from patients with asthma and chronic bronchitis were performed and found to be reproducible .
	manualset3
128170	3	405812	13	NULL	NULL	0	NULL	asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative sputum cell counts from patients with asthma and chronic bronchitis were performed and found to be reproducible .
	manualset3
128171	4	405812	13	NULL	NULL	0	NULL	chronic bronchitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative sputum cell counts from patients with asthma and chronic bronchitis were performed and found to be reproducible .
	manualset3
129474	1	405813	13	NULL	NULL	0	NULL	Quantitative studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative studies of color constancy .
	manualset3
129475	2	405813	13	NULL	NULL	0	NULL	color constancy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative studies of color constancy .
	manualset3
129476	1	405814	13	NULL	NULL	0	NULL	Quercetin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Quercetin induces cell death via apoptosis in both K562 and K562/adr cells and does not inhibit Pgp-mediated efflux of 99mTc-MIBI .
	manualset3
129477	2	405814	13	NULL	NULL	0	NULL	cell death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Quercetin induces cell death via apoptosis in both K562 and K562/adr cells and does not inhibit Pgp-mediated efflux of 99mTc-MIBI .
	manualset3
129478	3	405814	13	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Quercetin induces cell death via apoptosis in both K562 and K562/adr cells and does not inhibit Pgp-mediated efflux of 99mTc-MIBI .
	manualset3
129479	4	405814	13	NULL	NULL	0	NULL	K562 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Quercetin induces cell death via apoptosis in both K562 and K562/adr cells and does not inhibit Pgp-mediated efflux of 99mTc-MIBI .
	manualset3
129480	5	405814	13	NULL	NULL	0	NULL	K562/adr cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Quercetin induces cell death via apoptosis in both K562 and K562/adr cells and does not inhibit Pgp-mediated efflux of 99mTc-MIBI .
	manualset3
129481	6	405814	13	NULL	NULL	0	NULL	Pgp-mediated efflux 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Quercetin induces cell death via apoptosis in both K562 and K562/adr cells and does not inhibit Pgp-mediated efflux of 99mTc-MIBI .
	manualset3
129482	7	405814	13	NULL	NULL	0	NULL	99mTc-MIBI	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Quercetin induces cell death via apoptosis in both K562 and K562/adr cells and does not inhibit Pgp-mediated efflux of 99mTc-MIBI .
	manualset3
129483	1	405815	13	NULL	NULL	0	NULL	mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A mechanism for this action of these adrenal steroids has not been established , but it appears that the glucocorticoids influence LH release by acting on one or more post-receptor sites .
	manualset3
129484	2	405815	13	NULL	NULL	0	NULL	action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A mechanism for this action of these adrenal steroids has not been established , but it appears that the glucocorticoids influence LH release by acting on one or more post-receptor sites .
	manualset3
129485	3	405815	13	NULL	NULL	0	NULL	adrenal steroids 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A mechanism for this action of these adrenal steroids has not been established , but it appears that the glucocorticoids influence LH release by acting on one or more post-receptor sites .
	manualset3
129486	4	405815	13	NULL	NULL	0	NULL	glucocorticoids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A mechanism for this action of these adrenal steroids has not been established , but it appears that the glucocorticoids influence LH release by acting on one or more post-receptor sites .
	manualset3
129487	5	405815	13	NULL	NULL	0	NULL	LH release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A mechanism for this action of these adrenal steroids has not been established , but it appears that the glucocorticoids influence LH release by acting on one or more post-receptor sites .
	manualset3
129488	6	405815	13	NULL	NULL	0	NULL	post-receptor sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A mechanism for this action of these adrenal steroids has not been established , but it appears that the glucocorticoids influence LH release by acting on one or more post-receptor sites .
	manualset3
129489	1	405816	13	NULL	NULL	0	NULL	Quinacrine hydrochloride 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Quinacrine hydrochloride in the treatment of lupus erythematosus .
	manualset3
129490	2	405816	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Quinacrine hydrochloride in the treatment of lupus erythematosus .
	manualset3
129491	3	405816	13	NULL	NULL	0	NULL	lupus erythematosus 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Quinacrine hydrochloride in the treatment of lupus erythematosus .
	manualset3
129492	1	405817	13	NULL	NULL	0	NULL	R ( f ) values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	R ( f ) values of psoralen and daidzein were found to be 0.60 and 0.88 , whilst as their percentage values in methanolic extract were found to be 3.02 % and 5.64 % ( w/w ) , respectively .
	manualset3
129493	2	405817	13	NULL	NULL	0	NULL	psoralen	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	R ( f ) values of psoralen and daidzein were found to be 0.60 and 0.88 , whilst as their percentage values in methanolic extract were found to be 3.02 % and 5.64 % ( w/w ) , respectively .
	manualset3
129494	3	405817	13	NULL	NULL	0	NULL	daidzein	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	R ( f ) values of psoralen and daidzein were found to be 0.60 and 0.88 , whilst as their percentage values in methanolic extract were found to be 3.02 % and 5.64 % ( w/w ) , respectively .
	manualset3
129495	4	405817	13	NULL	NULL	0	NULL	0.60 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	R ( f ) values of psoralen and daidzein were found to be 0.60 and 0.88 , whilst as their percentage values in methanolic extract were found to be 3.02 % and 5.64 % ( w/w ) , respectively .
	manualset3
129496	5	405817	13	NULL	NULL	0	NULL	0.88	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	R ( f ) values of psoralen and daidzein were found to be 0.60 and 0.88 , whilst as their percentage values in methanolic extract were found to be 3.02 % and 5.64 % ( w/w ) , respectively .
	manualset3
129497	6	405817	13	NULL	NULL	0	NULL	percentage values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	R ( f ) values of psoralen and daidzein were found to be 0.60 and 0.88 , whilst as their percentage values in methanolic extract were found to be 3.02 % and 5.64 % ( w/w ) , respectively .
	manualset3
129498	7	405817	13	NULL	NULL	0	NULL	methanolic extract	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	R ( f ) values of psoralen and daidzein were found to be 0.60 and 0.88 , whilst as their percentage values in methanolic extract were found to be 3.02 % and 5.64 % ( w/w ) , respectively .
	manualset3
129499	8	405817	13	NULL	NULL	0	NULL	3.02 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	R ( f ) values of psoralen and daidzein were found to be 0.60 and 0.88 , whilst as their percentage values in methanolic extract were found to be 3.02 % and 5.64 % ( w/w ) , respectively .
	manualset3
129500	9	405817	13	NULL	NULL	0	NULL	5.64 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	R ( f ) values of psoralen and daidzein were found to be 0.60 and 0.88 , whilst as their percentage values in methanolic extract were found to be 3.02 % and 5.64 % ( w/w ) , respectively .
	manualset3
129501	1	405818	13	NULL	NULL	0	NULL	R12-2	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	R12-2 , a 62-base-pair , double-stranded DNA molecule with a monothio-phosphate modified backbone , was selected through a novel combinatorial selection method .
	manualset3
129502	2	405818	13	NULL	NULL	0	NULL	a 62-base-pair	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	R12-2 , a 62-base-pair , double-stranded DNA molecule with a monothio-phosphate modified backbone , was selected through a novel combinatorial selection method .
	manualset3
129503	3	405818	13	NULL	NULL	0	NULL	double-stranded DNA molecule	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	R12-2 , a 62-base-pair , double-stranded DNA molecule with a monothio-phosphate modified backbone , was selected through a novel combinatorial selection method .
	manualset3
129504	4	405818	13	NULL	NULL	NULL	NULL	monothio-phosphate modified backbone	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	R12-2 , a 62-base-pair , double-stranded DNA molecule with a monothio-phosphate modified backbone , was selected through a novel combinatorial selection method .
	manualset3
129505	5	405818	13	NULL	NULL	0	NULL	novel combinatorial selection method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	R12-2 , a 62-base-pair , double-stranded DNA molecule with a monothio-phosphate modified backbone , was selected through a novel combinatorial selection method .
	manualset3
129506	1	405819	13	NULL	NULL	0	NULL	R3Hs 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	R3Hs were mononuclear and of lower ploidy .
	manualset3
129507	2	405819	13	NULL	NULL	0	NULL	lower ploidy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	R3Hs were mononuclear and of lower ploidy .
	manualset3
129508	1	405820	13	NULL	NULL	0	NULL	RA-SF 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	RA-SF could , on the other hand , greatly enhance IL-2 production by CD4 + responder cells .
	manualset3
129509	2	405820	13	NULL	NULL	0	NULL	IL-2 production 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RA-SF could , on the other hand , greatly enhance IL-2 production by CD4 + responder cells .
	manualset3
129510	3	405820	13	NULL	NULL	0	NULL	CD4 + responder cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	RA-SF could , on the other hand , greatly enhance IL-2 production by CD4 + responder cells .
	manualset3
129511	1	405821	13	NULL	NULL	0	NULL	RAD51	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	RAD51 is an essential enzyme for the homologous recombinational repair ( HRR ) of DNA double-strand breaks .
	manualset3
129512	2	405821	13	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	RAD51 is an essential enzyme for the homologous recombinational repair ( HRR ) of DNA double-strand breaks .
	manualset3
129513	3	405821	13	NULL	NULL	0	NULL	homologous recombinational repair ( HRR )	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RAD51 is an essential enzyme for the homologous recombinational repair ( HRR ) of DNA double-strand breaks .
	manualset3
129514	4	405821	13	NULL	NULL	0	NULL	DNA double-strand breaks	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RAD51 is an essential enzyme for the homologous recombinational repair ( HRR ) of DNA double-strand breaks .
	manualset3
129515	1	405822	13	NULL	NULL	0	NULL	mechanism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A mechanism is proposed which accounts for the origin of the selectivity changes .
	manualset3
129516	2	405822	13	NULL	NULL	0	NULL	origin	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A mechanism is proposed which accounts for the origin of the selectivity changes .
	manualset3
129517	3	405822	13	NULL	NULL	0	NULL	selectivity changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A mechanism is proposed which accounts for the origin of the selectivity changes .
	manualset3
129518	1	405823	13	NULL	NULL	0	NULL	RAGE	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	RAGE opposes Myd88 signaling at multiple levels : by suppression of p65 levels , thereby reducing activation of NF-B and consequent production of cyclin D1 , and by suppression of Il6-mediated phosphorylation of Stat3 , thereby down-regulating Pim1 and suppressing the hyperplastic response .
	manualset3
129519	2	405823	13	NULL	NULL	0	NULL	Myd88 signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RAGE opposes Myd88 signaling at multiple levels : by suppression of p65 levels , thereby reducing activation of NF-B and consequent production of cyclin D1 , and by suppression of Il6-mediated phosphorylation of Stat3 , thereby down-regulating Pim1 and suppressing the hyperplastic response .
	manualset3
129520	3	405823	13	NULL	NULL	0	NULL	levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	RAGE opposes Myd88 signaling at multiple levels : by suppression of p65 levels , thereby reducing activation of NF-B and consequent production of cyclin D1 , and by suppression of Il6-mediated phosphorylation of Stat3 , thereby down-regulating Pim1 and suppressing the hyperplastic response .
	manualset3
129521	4	405823	13	NULL	NULL	0	NULL	suppression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RAGE opposes Myd88 signaling at multiple levels : by suppression of p65 levels , thereby reducing activation of NF-B and consequent production of cyclin D1 , and by suppression of Il6-mediated phosphorylation of Stat3 , thereby down-regulating Pim1 and suppressing the hyperplastic response .
	manualset3
129522	5	405823	13	NULL	NULL	0	NULL	p65 levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	RAGE opposes Myd88 signaling at multiple levels : by suppression of p65 levels , thereby reducing activation of NF-B and consequent production of cyclin D1 , and by suppression of Il6-mediated phosphorylation of Stat3 , thereby down-regulating Pim1 and suppressing the hyperplastic response .
	manualset3
129523	6	405823	13	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RAGE opposes Myd88 signaling at multiple levels : by suppression of p65 levels , thereby reducing activation of NF-B and consequent production of cyclin D1 , and by suppression of Il6-mediated phosphorylation of Stat3 , thereby down-regulating Pim1 and suppressing the hyperplastic response .
	manualset3
129524	7	405823	13	NULL	NULL	0	NULL	NF-B 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	RAGE opposes Myd88 signaling at multiple levels : by suppression of p65 levels , thereby reducing activation of NF-B and consequent production of cyclin D1 , and by suppression of Il6-mediated phosphorylation of Stat3 , thereby down-regulating Pim1 and suppressing the hyperplastic response .
	manualset3
129525	8	405823	13	NULL	NULL	0	NULL	production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RAGE opposes Myd88 signaling at multiple levels : by suppression of p65 levels , thereby reducing activation of NF-B and consequent production of cyclin D1 , and by suppression of Il6-mediated phosphorylation of Stat3 , thereby down-regulating Pim1 and suppressing the hyperplastic response .
	manualset3
129526	9	405823	13	NULL	NULL	0	NULL	cyclin D1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	RAGE opposes Myd88 signaling at multiple levels : by suppression of p65 levels , thereby reducing activation of NF-B and consequent production of cyclin D1 , and by suppression of Il6-mediated phosphorylation of Stat3 , thereby down-regulating Pim1 and suppressing the hyperplastic response .
	manualset3
129527	10	405823	13	NULL	NULL	0	NULL	suppression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RAGE opposes Myd88 signaling at multiple levels : by suppression of p65 levels , thereby reducing activation of NF-B and consequent production of cyclin D1 , and by suppression of Il6-mediated phosphorylation of Stat3 , thereby down-regulating Pim1 and suppressing the hyperplastic response .
	manualset3
129528	11	405823	13	NULL	NULL	0	NULL	Il6-mediated phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RAGE opposes Myd88 signaling at multiple levels : by suppression of p65 levels , thereby reducing activation of NF-B and consequent production of cyclin D1 , and by suppression of Il6-mediated phosphorylation of Stat3 , thereby down-regulating Pim1 and suppressing the hyperplastic response .
	manualset3
129529	12	405823	13	NULL	NULL	0	NULL	Stat3 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	RAGE opposes Myd88 signaling at multiple levels : by suppression of p65 levels , thereby reducing activation of NF-B and consequent production of cyclin D1 , and by suppression of Il6-mediated phosphorylation of Stat3 , thereby down-regulating Pim1 and suppressing the hyperplastic response .
	manualset3
129530	13	405823	13	NULL	NULL	0	NULL	Pim1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	RAGE opposes Myd88 signaling at multiple levels : by suppression of p65 levels , thereby reducing activation of NF-B and consequent production of cyclin D1 , and by suppression of Il6-mediated phosphorylation of Stat3 , thereby down-regulating Pim1 and suppressing the hyperplastic response .
	manualset3
129531	14	405823	13	NULL	NULL	0	NULL	hyperplastic response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RAGE opposes Myd88 signaling at multiple levels : by suppression of p65 levels , thereby reducing activation of NF-B and consequent production of cyclin D1 , and by suppression of Il6-mediated phosphorylation of Stat3 , thereby down-regulating Pim1 and suppressing the hyperplastic response .
	manualset3
129532	1	405824	13	NULL	NULL	0	NULL	RANKL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	RANKL and RANK ( coded for by the TNFRSF11A gene ) also play a role in the immune system , which raises the possibility that defects in this pathway might cause osteopetrosis with immunodeficiency .
	manualset3
129533	2	405824	13	NULL	NULL	0	NULL	RANK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	RANKL and RANK ( coded for by the TNFRSF11A gene ) also play a role in the immune system , which raises the possibility that defects in this pathway might cause osteopetrosis with immunodeficiency .
	manualset3
129534	3	405824	13	NULL	NULL	0	NULL	TNFRSF11A gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	RANKL and RANK ( coded for by the TNFRSF11A gene ) also play a role in the immune system , which raises the possibility that defects in this pathway might cause osteopetrosis with immunodeficiency .
	manualset3
129535	4	405824	13	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RANKL and RANK ( coded for by the TNFRSF11A gene ) also play a role in the immune system , which raises the possibility that defects in this pathway might cause osteopetrosis with immunodeficiency .
	manualset3
129536	5	405824	13	NULL	NULL	0	NULL	immune system 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RANKL and RANK ( coded for by the TNFRSF11A gene ) also play a role in the immune system , which raises the possibility that defects in this pathway might cause osteopetrosis with immunodeficiency .
	manualset3
129537	6	405824	13	NULL	NULL	0	NULL	possibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	RANKL and RANK ( coded for by the TNFRSF11A gene ) also play a role in the immune system , which raises the possibility that defects in this pathway might cause osteopetrosis with immunodeficiency .
	manualset3
129538	7	405824	13	NULL	NULL	0	NULL	defects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RANKL and RANK ( coded for by the TNFRSF11A gene ) also play a role in the immune system , which raises the possibility that defects in this pathway might cause osteopetrosis with immunodeficiency .
	manualset3
129539	8	405824	13	NULL	NULL	0	NULL	pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RANKL and RANK ( coded for by the TNFRSF11A gene ) also play a role in the immune system , which raises the possibility that defects in this pathway might cause osteopetrosis with immunodeficiency .
	manualset3
129540	9	405824	13	NULL	NULL	0	NULL	osteopetrosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	RANKL and RANK ( coded for by the TNFRSF11A gene ) also play a role in the immune system , which raises the possibility that defects in this pathway might cause osteopetrosis with immunodeficiency .
	manualset3
129541	10	405824	13	NULL	NULL	0	NULL	immunodeficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	RANKL and RANK ( coded for by the TNFRSF11A gene ) also play a role in the immune system , which raises the possibility that defects in this pathway might cause osteopetrosis with immunodeficiency .
	manualset3
129542	1	405825	13	NULL	NULL	0	NULL	RASMCs 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	RASMCs were exposed to uniaxial CS and thereafter collected to evaluate the expressions of mRNA or protein relating aldosterone synthesis and the nicotinamide adenine dinucleotide phosphate ( NADPH ) oxidase activity .
	manualset3
129543	2	405825	13	NULL	NULL	0	NULL	uniaxial CS	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RASMCs were exposed to uniaxial CS and thereafter collected to evaluate the expressions of mRNA or protein relating aldosterone synthesis and the nicotinamide adenine dinucleotide phosphate ( NADPH ) oxidase activity .
	manualset3
129544	3	405825	13	NULL	NULL	0	NULL	expressions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RASMCs were exposed to uniaxial CS and thereafter collected to evaluate the expressions of mRNA or protein relating aldosterone synthesis and the nicotinamide adenine dinucleotide phosphate ( NADPH ) oxidase activity .
	manualset3
129545	4	405825	13	NULL	NULL	0	NULL	mRNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	RASMCs were exposed to uniaxial CS and thereafter collected to evaluate the expressions of mRNA or protein relating aldosterone synthesis and the nicotinamide adenine dinucleotide phosphate ( NADPH ) oxidase activity .
	manualset3
129546	5	405825	13	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	RASMCs were exposed to uniaxial CS and thereafter collected to evaluate the expressions of mRNA or protein relating aldosterone synthesis and the nicotinamide adenine dinucleotide phosphate ( NADPH ) oxidase activity .
	manualset3
129547	6	405825	13	NULL	NULL	0	NULL	aldosterone synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RASMCs were exposed to uniaxial CS and thereafter collected to evaluate the expressions of mRNA or protein relating aldosterone synthesis and the nicotinamide adenine dinucleotide phosphate ( NADPH ) oxidase activity .
	manualset3
129548	7	405825	13	NULL	NULL	0	NULL	nicotinamide adenine dinucleotide phosphate ( NADPH ) oxidase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RASMCs were exposed to uniaxial CS and thereafter collected to evaluate the expressions of mRNA or protein relating aldosterone synthesis and the nicotinamide adenine dinucleotide phosphate ( NADPH ) oxidase activity .
	manualset3
129549	1	405826	13	NULL	NULL	0	NULL	RB18A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	RB18A , whose gene is localized on chromosome 17q12-q21 .1 , regulates in vivo p53 transactivating activity .
	manualset3
129550	2	405826	13	NULL	NULL	0	NULL	gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	RB18A , whose gene is localized on chromosome 17q12-q21 .1 , regulates in vivo p53 transactivating activity .
	manualset3
129551	3	405826	13	NULL	NULL	0	NULL	chromosome 17q12-q21 .1	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	RB18A , whose gene is localized on chromosome 17q12-q21 .1 , regulates in vivo p53 transactivating activity .
	manualset3
129552	4	405826	13	NULL	NULL	0	NULL	regulates 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RB18A , whose gene is localized on chromosome 17q12-q21 .1 , regulates in vivo p53 transactivating activity .
	manualset3
129553	5	405826	13	NULL	NULL	0	NULL	p53 transactivating activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RB18A , whose gene is localized on chromosome 17q12-q21 .1 , regulates in vivo p53 transactivating activity .
	manualset3
129554	1	405827	13	NULL	NULL	0	NULL	RCE1 corneal epithelial cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	RCE1 corneal epithelial cell line : its variability on phenotype expression and differential response to growth factors .
	manualset3
129555	2	405827	13	NULL	NULL	0	NULL	variability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RCE1 corneal epithelial cell line : its variability on phenotype expression and differential response to growth factors .
	manualset3
129556	3	405827	13	NULL	NULL	NULL	NULL	phenotype expression	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	RCE1 corneal epithelial cell line : its variability on phenotype expression and differential response to growth factors .
	manualset3
129557	4	405827	13	NULL	NULL	0	NULL	differential response 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RCE1 corneal epithelial cell line : its variability on phenotype expression and differential response to growth factors .
	manualset3
129558	5	405827	13	NULL	NULL	0	NULL	growth factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	RCE1 corneal epithelial cell line : its variability on phenotype expression and differential response to growth factors .
	manualset3
129559	1	405828	13	NULL	NULL	0	NULL	REHABILITATION 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	REHABILITATION OF SEVERELY HANDICAPPED PATIENTS IN SWEDEN : METHODS AND MEDICAL , SOCIAL AND ECONOMIC RESULTS .
	manualset3
129560	2	405828	13	NULL	NULL	0	NULL	SEVERELY HANDICAPPED PATIENTS	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	REHABILITATION OF SEVERELY HANDICAPPED PATIENTS IN SWEDEN : METHODS AND MEDICAL , SOCIAL AND ECONOMIC RESULTS .
	manualset3
129561	3	405828	13	NULL	NULL	0	NULL	SWEDEN 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	REHABILITATION OF SEVERELY HANDICAPPED PATIENTS IN SWEDEN : METHODS AND MEDICAL , SOCIAL AND ECONOMIC RESULTS .
	manualset3
129562	4	405828	13	NULL	NULL	NULL	NULL	METHODS AND MEDICAL RESULTS 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	REHABILITATION OF SEVERELY HANDICAPPED PATIENTS IN SWEDEN : METHODS AND MEDICAL , SOCIAL AND ECONOMIC RESULTS .
	manualset3
129563	5	405828	13	NULL	NULL	0	NULL	SOCIAL AND ECONOMIC RESULTS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	REHABILITATION OF SEVERELY HANDICAPPED PATIENTS IN SWEDEN : METHODS AND MEDICAL , SOCIAL AND ECONOMIC RESULTS .
	manualset3
129564	1	405829	13	NULL	NULL	0	NULL	RESULTS	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	RESULTS : ISPyB is now a multisite , generic LIMS for synchrotron-based MX experiments .
	manualset3
129565	2	405829	13	NULL	NULL	0	NULL	ISPyB	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	RESULTS : ISPyB is now a multisite , generic LIMS for synchrotron-based MX experiments .
	manualset3
129566	3	405829	13	NULL	NULL	0	NULL	multisite	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	RESULTS : ISPyB is now a multisite , generic LIMS for synchrotron-based MX experiments .
	manualset3
129567	4	405829	13	NULL	NULL	0	NULL	generic LIMS 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	RESULTS : ISPyB is now a multisite , generic LIMS for synchrotron-based MX experiments .
	manualset3
129568	5	405829	13	NULL	NULL	0	NULL	synchrotron-based MX experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	RESULTS : ISPyB is now a multisite , generic LIMS for synchrotron-based MX experiments .
	manualset3
129569	1	405830	13	NULL	NULL	0	NULL	mechanistic model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A mechanistic model for fate and removal of estrogens in biological nutrient removal activated sludge systems .
	manualset3
129570	2	405830	13	NULL	NULL	NULL	NULL	fate	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A mechanistic model for fate and removal of estrogens in biological nutrient removal activated sludge systems .
	manualset3
129571	3	405830	13	NULL	NULL	NULL	NULL	removal	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A mechanistic model for fate and removal of estrogens in biological nutrient removal activated sludge systems .
	manualset3
129572	4	405830	13	NULL	NULL	0	NULL	estrogens	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A mechanistic model for fate and removal of estrogens in biological nutrient removal activated sludge systems .
	manualset3
129573	5	405830	13	NULL	NULL	0	NULL	biological nutrient removal activated sludge systems	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A mechanistic model for fate and removal of estrogens in biological nutrient removal activated sludge systems .
	manualset3
128172	1	405831	13	NULL	NULL	0	NULL	RESULTS 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	RESULTS We found that primate ovarian tissue can be maintained for up to 24 h at 4C without compromising tissue or follicle health .
	manualset3
128173	2	405831	13	NULL	NULL	0	NULL	primate ovarian tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	RESULTS We found that primate ovarian tissue can be maintained for up to 24 h at 4C without compromising tissue or follicle health .
	manualset3
128174	3	405831	13	NULL	NULL	0	NULL	24 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	RESULTS We found that primate ovarian tissue can be maintained for up to 24 h at 4C without compromising tissue or follicle health .
	manualset3
128175	4	405831	13	NULL	NULL	0	NULL	4C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	RESULTS We found that primate ovarian tissue can be maintained for up to 24 h at 4C without compromising tissue or follicle health .
	manualset3
128176	5	405831	13	NULL	NULL	0	NULL	tissue 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	RESULTS We found that primate ovarian tissue can be maintained for up to 24 h at 4C without compromising tissue or follicle health .
	manualset3
128177	6	405831	13	NULL	NULL	0	NULL	follicle health 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	RESULTS We found that primate ovarian tissue can be maintained for up to 24 h at 4C without compromising tissue or follicle health .
	manualset3
128178	1	405832	13	NULL	NULL	0	NULL	REVIEW METHOD	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	REVIEW METHOD : The basic search process included a systematic review of articles contained in the PubMed/Medline database , dating between 1990 and 2005 , using single or combined key words to obtain the most comprehensive list of references ; a perusal of the references of the references completed the review .
	manualset3
128179	2	405832	13	NULL	NULL	0	NULL	search process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	REVIEW METHOD : The basic search process included a systematic review of articles contained in the PubMed/Medline database , dating between 1990 and 2005 , using single or combined key words to obtain the most comprehensive list of references ; a perusal of the references of the references completed the review .
	manualset3
128180	3	405832	13	NULL	NULL	0	NULL	systematic review	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	REVIEW METHOD : The basic search process included a systematic review of articles contained in the PubMed/Medline database , dating between 1990 and 2005 , using single or combined key words to obtain the most comprehensive list of references ; a perusal of the references of the references completed the review .
	manualset3
128181	4	405832	13	NULL	NULL	0	NULL	articles 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	REVIEW METHOD : The basic search process included a systematic review of articles contained in the PubMed/Medline database , dating between 1990 and 2005 , using single or combined key words to obtain the most comprehensive list of references ; a perusal of the references of the references completed the review .
	manualset3
128182	5	405832	13	NULL	NULL	0	NULL	PubMed/Medline database	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	REVIEW METHOD : The basic search process included a systematic review of articles contained in the PubMed/Medline database , dating between 1990 and 2005 , using single or combined key words to obtain the most comprehensive list of references ; a perusal of the references of the references completed the review .
	manualset3
128183	6	405832	13	NULL	NULL	0	NULL	1990	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	REVIEW METHOD : The basic search process included a systematic review of articles contained in the PubMed/Medline database , dating between 1990 and 2005 , using single or combined key words to obtain the most comprehensive list of references ; a perusal of the references of the references completed the review .
	manualset3
128184	7	405832	13	NULL	NULL	0	NULL	2005	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	REVIEW METHOD : The basic search process included a systematic review of articles contained in the PubMed/Medline database , dating between 1990 and 2005 , using single or combined key words to obtain the most comprehensive list of references ; a perusal of the references of the references completed the review .
	manualset3
128185	8	405832	13	NULL	NULL	0	NULL	key words	Language												NULL		0	NULL	NULL	NULL	NULL	NULL	REVIEW METHOD : The basic search process included a systematic review of articles contained in the PubMed/Medline database , dating between 1990 and 2005 , using single or combined key words to obtain the most comprehensive list of references ; a perusal of the references of the references completed the review .
	manualset3
128186	9	405832	13	NULL	NULL	0	NULL	comprehensive list of references	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	REVIEW METHOD : The basic search process included a systematic review of articles contained in the PubMed/Medline database , dating between 1990 and 2005 , using single or combined key words to obtain the most comprehensive list of references ; a perusal of the references of the references completed the review .
	manualset3
128187	10	405832	13	NULL	NULL	0	NULL	perusal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	REVIEW METHOD : The basic search process included a systematic review of articles contained in the PubMed/Medline database , dating between 1990 and 2005 , using single or combined key words to obtain the most comprehensive list of references ; a perusal of the references of the references completed the review .
	manualset3
128188	11	405832	13	NULL	NULL	0	NULL	references 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	REVIEW METHOD : The basic search process included a systematic review of articles contained in the PubMed/Medline database , dating between 1990 and 2005 , using single or combined key words to obtain the most comprehensive list of references ; a perusal of the references of the references completed the review .
	manualset3
128189	12	405832	13	NULL	NULL	0	NULL	references	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	REVIEW METHOD : The basic search process included a systematic review of articles contained in the PubMed/Medline database , dating between 1990 and 2005 , using single or combined key words to obtain the most comprehensive list of references ; a perusal of the references of the references completed the review .
	manualset3
128190	13	405832	13	NULL	NULL	0	NULL	review	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	REVIEW METHOD : The basic search process included a systematic review of articles contained in the PubMed/Medline database , dating between 1990 and 2005 , using single or combined key words to obtain the most comprehensive list of references ; a perusal of the references of the references completed the review .
	manualset3
128191	1	405833	13	NULL	NULL	0	NULL	RFs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	RFs also have been demonstrated to react with two different regions , SKDWSFY and LSQPKIVKWDR , on beta 2-microglobulin ( beta 2m ) .
	manualset3
128192	2	405833	13	NULL	NULL	0	NULL	two different regions 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	RFs also have been demonstrated to react with two different regions , SKDWSFY and LSQPKIVKWDR , on beta 2-microglobulin ( beta 2m ) .
	manualset3
128193	3	405833	13	NULL	NULL	0	NULL	SKDWSFY 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	RFs also have been demonstrated to react with two different regions , SKDWSFY and LSQPKIVKWDR , on beta 2-microglobulin ( beta 2m ) .
	manualset3
128194	4	405833	13	NULL	NULL	0	NULL	LSQPKIVKWDR 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	RFs also have been demonstrated to react with two different regions , SKDWSFY and LSQPKIVKWDR , on beta 2-microglobulin ( beta 2m ) .
	manualset3
128195	5	405833	13	NULL	NULL	0	NULL	beta 2-microglobulin ( beta 2m )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	RFs also have been demonstrated to react with two different regions , SKDWSFY and LSQPKIVKWDR , on beta 2-microglobulin ( beta 2m ) .
	manualset3
128196	1	405834	13	NULL	NULL	0	NULL	RGS2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	RGS2 decreases cAMP production and appears to interact with both adenylyl cyclase ( AC ) and its stimulatory G protein Gs .
	manualset3
128197	2	405834	13	NULL	NULL	0	NULL	cAMP production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RGS2 decreases cAMP production and appears to interact with both adenylyl cyclase ( AC ) and its stimulatory G protein Gs .
	manualset3
128198	3	405834	13	NULL	NULL	0	NULL	adenylyl cyclase ( AC )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	RGS2 decreases cAMP production and appears to interact with both adenylyl cyclase ( AC ) and its stimulatory G protein Gs .
	manualset3
128199	4	405834	13	NULL	NULL	0	NULL	stimulatory G protein Gs 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	RGS2 decreases cAMP production and appears to interact with both adenylyl cyclase ( AC ) and its stimulatory G protein Gs .
	manualset3
128200	1	405835	13	NULL	NULL	0	NULL	RHAMM peptides-analytic tools	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	RHAMM and CD44 peptides-analytic tools and potential drugs .
	manualset3
128201	2	405835	13	NULL	NULL	0	NULL	CD44 peptides-analytic tools	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	RHAMM and CD44 peptides-analytic tools and potential drugs .
	manualset3
128202	3	405835	13	NULL	NULL	0	NULL	potential drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	RHAMM and CD44 peptides-analytic tools and potential drugs .
	manualset3
128203	1	405836	13	NULL	NULL	0	NULL	RIS	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	RIS dose-dependently inhibited prenylation of both Rap1A and Rab6 , whereas 3-PEHPC only inhibited Rab6 prenylation .
	manualset3
128204	2	405836	13	NULL	NULL	0	NULL	prenylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RIS dose-dependently inhibited prenylation of both Rap1A and Rab6 , whereas 3-PEHPC only inhibited Rab6 prenylation .
	manualset3
128205	3	405836	13	NULL	NULL	0	NULL	Rap1A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	RIS dose-dependently inhibited prenylation of both Rap1A and Rab6 , whereas 3-PEHPC only inhibited Rab6 prenylation .
	manualset3
128206	4	405836	13	NULL	NULL	0	NULL	Rab6 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	RIS dose-dependently inhibited prenylation of both Rap1A and Rab6 , whereas 3-PEHPC only inhibited Rab6 prenylation .
	manualset3
128207	5	405836	13	NULL	NULL	0	NULL	3-PEHPC 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	RIS dose-dependently inhibited prenylation of both Rap1A and Rab6 , whereas 3-PEHPC only inhibited Rab6 prenylation .
	manualset3
128208	6	405836	13	NULL	NULL	0	NULL	Rab6 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	RIS dose-dependently inhibited prenylation of both Rap1A and Rab6 , whereas 3-PEHPC only inhibited Rab6 prenylation .
	manualset3
128209	7	405836	13	NULL	NULL	0	NULL	prenylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RIS dose-dependently inhibited prenylation of both Rap1A and Rab6 , whereas 3-PEHPC only inhibited Rab6 prenylation .
	manualset3
128210	1	405837	13	NULL	NULL	0	NULL	RIT 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	RIT using alpha-emitters such as ( 213 ) Bi , ( 211 ) At , ( 225 ) Ac , and others has demonstrated significant activity in both in vitro and in vivo model systems .
	manualset3
128211	2	405837	13	NULL	NULL	0	NULL	alpha-emitters	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	RIT using alpha-emitters such as ( 213 ) Bi , ( 211 ) At , ( 225 ) Ac , and others has demonstrated significant activity in both in vitro and in vivo model systems .
	manualset3
128212	3	405837	13	NULL	NULL	0	NULL	( 213 ) Bi	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	RIT using alpha-emitters such as ( 213 ) Bi , ( 211 ) At , ( 225 ) Ac , and others has demonstrated significant activity in both in vitro and in vivo model systems .
	manualset3
128213	4	405837	13	NULL	NULL	0	NULL	( 211 ) At	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	RIT using alpha-emitters such as ( 213 ) Bi , ( 211 ) At , ( 225 ) Ac , and others has demonstrated significant activity in both in vitro and in vivo model systems .
	manualset3
128214	5	405837	13	NULL	NULL	0	NULL	( 225 ) Ac	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	RIT using alpha-emitters such as ( 213 ) Bi , ( 211 ) At , ( 225 ) Ac , and others has demonstrated significant activity in both in vitro and in vivo model systems .
	manualset3
128215	6	405837	13	NULL	NULL	0	NULL	activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	RIT using alpha-emitters such as ( 213 ) Bi , ( 211 ) At , ( 225 ) Ac , and others has demonstrated significant activity in both in vitro and in vivo model systems .
	manualset3
128216	7	405837	13	NULL	NULL	0	NULL	model systems	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	RIT using alpha-emitters such as ( 213 ) Bi , ( 211 ) At , ( 225 ) Ac , and others has demonstrated significant activity in both in vitro and in vivo model systems .
	manualset3
128217	1	405838	13	NULL	NULL	0	NULL	RMI 12 , 936	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	RMI 12 , 936 , when injected subcutaneously at a dose of 2 mg , either on Day 6 of psuedopregnancy ( PSP-6 ) or on PSP-6 , 7 and 8 , shortened the duration of PSP from 12.3 + / - 0.3 ( control ) to 8.3 + / - 0.1 or 8.7 + / - 0.2 days , respectively .
	manualset3
128218	2	405838	13	NULL	NULL	0	NULL	dose of 2 mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	RMI 12 , 936 , when injected subcutaneously at a dose of 2 mg , either on Day 6 of psuedopregnancy ( PSP-6 ) or on PSP-6 , 7 and 8 , shortened the duration of PSP from 12.3 + / - 0.3 ( control ) to 8.3 + / - 0.1 or 8.7 + / - 0.2 days , respectively .
	manualset3
128219	3	405838	13	NULL	NULL	0	NULL	Day 6 of psuedopregnancy ( PSP-6 ) 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	RMI 12 , 936 , when injected subcutaneously at a dose of 2 mg , either on Day 6 of psuedopregnancy ( PSP-6 ) or on PSP-6 , 7 and 8 , shortened the duration of PSP from 12.3 + / - 0.3 ( control ) to 8.3 + / - 0.1 or 8.7 + / - 0.2 days , respectively .
	manualset3
128220	4	405838	13	NULL	NULL	0	NULL	PSP-6	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	RMI 12 , 936 , when injected subcutaneously at a dose of 2 mg , either on Day 6 of psuedopregnancy ( PSP-6 ) or on PSP-6 , 7 and 8 , shortened the duration of PSP from 12.3 + / - 0.3 ( control ) to 8.3 + / - 0.1 or 8.7 + / - 0.2 days , respectively .
	manualset3
128221	5	405838	13	NULL	NULL	0	NULL	PSP-7													NULL		0	NULL	NULL	NULL	NULL	NULL	RMI 12 , 936 , when injected subcutaneously at a dose of 2 mg , either on Day 6 of psuedopregnancy ( PSP-6 ) or on PSP-6 , 7 and 8 , shortened the duration of PSP from 12.3 + / - 0.3 ( control ) to 8.3 + / - 0.1 or 8.7 + / - 0.2 days , respectively .
	manualset3
128222	6	405838	13	NULL	NULL	0	NULL	PSP-8	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	RMI 12 , 936 , when injected subcutaneously at a dose of 2 mg , either on Day 6 of psuedopregnancy ( PSP-6 ) or on PSP-6 , 7 and 8 , shortened the duration of PSP from 12.3 + / - 0.3 ( control ) to 8.3 + / - 0.1 or 8.7 + / - 0.2 days , respectively .
	manualset3
128223	7	405838	13	NULL	NULL	0	NULL	duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	RMI 12 , 936 , when injected subcutaneously at a dose of 2 mg , either on Day 6 of psuedopregnancy ( PSP-6 ) or on PSP-6 , 7 and 8 , shortened the duration of PSP from 12.3 + / - 0.3 ( control ) to 8.3 + / - 0.1 or 8.7 + / - 0.2 days , respectively .
	manualset3
128224	8	405838	13	NULL	NULL	0	NULL	PSP	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	RMI 12 , 936 , when injected subcutaneously at a dose of 2 mg , either on Day 6 of psuedopregnancy ( PSP-6 ) or on PSP-6 , 7 and 8 , shortened the duration of PSP from 12.3 + / - 0.3 ( control ) to 8.3 + / - 0.1 or 8.7 + / - 0.2 days , respectively .
	manualset3
128225	9	405838	13	NULL	NULL	0	NULL	12.3 + / - 0.3 ( control ) to 8.3 + / - 0.1 days	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	RMI 12 , 936 , when injected subcutaneously at a dose of 2 mg , either on Day 6 of psuedopregnancy ( PSP-6 ) or on PSP-6 , 7 and 8 , shortened the duration of PSP from 12.3 + / - 0.3 ( control ) to 8.3 + / - 0.1 or 8.7 + / - 0.2 days , respectively .
	manualset3
128226	10	405838	13	NULL	NULL	NULL	NULL	12.3 + / - 0.3 ( control ) to 8.7 + / - 0.2 days 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	RMI 12 , 936 , when injected subcutaneously at a dose of 2 mg , either on Day 6 of psuedopregnancy ( PSP-6 ) or on PSP-6 , 7 and 8 , shortened the duration of PSP from 12.3 + / - 0.3 ( control ) to 8.3 + / - 0.1 or 8.7 + / - 0.2 days , respectively .
	manualset3
128227	1	405839	13	NULL	NULL	0	NULL	RNA editing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	RNA editing at the Q/R site for the glutamate receptor subunits GLUR2 , GLUR5 , and GLUR6 in hippocampus and temporal cortex from epileptic patients .
	manualset3
128228	2	405839	13	NULL	NULL	0	NULL	Q/R site	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	RNA editing at the Q/R site for the glutamate receptor subunits GLUR2 , GLUR5 , and GLUR6 in hippocampus and temporal cortex from epileptic patients .
	manualset3
128229	3	405839	13	NULL	NULL	0	NULL	glutamate receptor subunits	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	RNA editing at the Q/R site for the glutamate receptor subunits GLUR2 , GLUR5 , and GLUR6 in hippocampus and temporal cortex from epileptic patients .
	manualset3
128230	4	405839	13	NULL	NULL	0	NULL	GLUR2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	RNA editing at the Q/R site for the glutamate receptor subunits GLUR2 , GLUR5 , and GLUR6 in hippocampus and temporal cortex from epileptic patients .
	manualset3
128231	5	405839	13	NULL	NULL	0	NULL	GLUR5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	RNA editing at the Q/R site for the glutamate receptor subunits GLUR2 , GLUR5 , and GLUR6 in hippocampus and temporal cortex from epileptic patients .
	manualset3
128232	6	405839	13	NULL	NULL	0	NULL	GLUR6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	RNA editing at the Q/R site for the glutamate receptor subunits GLUR2 , GLUR5 , and GLUR6 in hippocampus and temporal cortex from epileptic patients .
	manualset3
128233	7	405839	13	NULL	NULL	0	NULL	hippocampus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	RNA editing at the Q/R site for the glutamate receptor subunits GLUR2 , GLUR5 , and GLUR6 in hippocampus and temporal cortex from epileptic patients .
	manualset3
128234	8	405839	13	NULL	NULL	0	NULL	temporal cortex 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	RNA editing at the Q/R site for the glutamate receptor subunits GLUR2 , GLUR5 , and GLUR6 in hippocampus and temporal cortex from epileptic patients .
	manualset3
128235	9	405839	13	NULL	NULL	0	NULL	epileptic patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	RNA editing at the Q/R site for the glutamate receptor subunits GLUR2 , GLUR5 , and GLUR6 in hippocampus and temporal cortex from epileptic patients .
	manualset3
128236	1	405840	13	NULL	NULL	0	NULL	RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	RNA has been shown to bind to the N-terminal domain ( NTD ) , although recently the C-terminal half of the protein has also been implicated in RNA binding .
	manualset3
128237	2	405840	13	NULL	NULL	0	NULL	 N-terminal domain ( NTD ) 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	RNA has been shown to bind to the N-terminal domain ( NTD ) , although recently the C-terminal half of the protein has also been implicated in RNA binding .
	manualset3
128238	3	405840	13	NULL	NULL	0	NULL	C-terminal half 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	RNA has been shown to bind to the N-terminal domain ( NTD ) , although recently the C-terminal half of the protein has also been implicated in RNA binding .
	manualset3
128239	4	405840	13	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	RNA has been shown to bind to the N-terminal domain ( NTD ) , although recently the C-terminal half of the protein has also been implicated in RNA binding .
	manualset3
128240	5	405840	13	NULL	NULL	0	NULL	RNA binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RNA has been shown to bind to the N-terminal domain ( NTD ) , although recently the C-terminal half of the protein has also been implicated in RNA binding .
	manualset3
128241	1	405841	13	NULL	NULL	NULL	NULL	RNase-treatment	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	RNase-treatment , but not proteinase K-treatment destroyed the protective properties of fraction II , and RNA purified from fraction II also induced protection .
	manualset3
128242	2	405841	13	NULL	NULL	0	NULL	proteinase K-treatment 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RNase-treatment , but not proteinase K-treatment destroyed the protective properties of fraction II , and RNA purified from fraction II also induced protection .
	manualset3
128243	3	405841	13	NULL	NULL	0	NULL	protective properties	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RNase-treatment , but not proteinase K-treatment destroyed the protective properties of fraction II , and RNA purified from fraction II also induced protection .
	manualset3
128244	4	405841	13	NULL	NULL	0	NULL	fraction II	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	RNase-treatment , but not proteinase K-treatment destroyed the protective properties of fraction II , and RNA purified from fraction II also induced protection .
	manualset3
128245	5	405841	13	NULL	NULL	0	NULL	RNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	RNase-treatment , but not proteinase K-treatment destroyed the protective properties of fraction II , and RNA purified from fraction II also induced protection .
	manualset3
128246	6	405841	13	NULL	NULL	0	NULL	fraction II 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	RNase-treatment , but not proteinase K-treatment destroyed the protective properties of fraction II , and RNA purified from fraction II also induced protection .
	manualset3
128247	7	405841	13	NULL	NULL	0	NULL	protection 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RNase-treatment , but not proteinase K-treatment destroyed the protective properties of fraction II , and RNA purified from fraction II also induced protection .
	manualset3
128248	1	405842	13	NULL	NULL	0	NULL	ROCK 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	ROCK : the Roche medicinal chemistry knowledge application - design , use and impact .
	manualset3
128249	2	405842	13	NULL	NULL	0	NULL	Roche medicinal chemistry knowledge application	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	ROCK : the Roche medicinal chemistry knowledge application - design , use and impact .
	manualset3
128250	3	405842	13	NULL	NULL	0	NULL	design	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	ROCK : the Roche medicinal chemistry knowledge application - design , use and impact .
	manualset3
128251	4	405842	13	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	ROCK : the Roche medicinal chemistry knowledge application - design , use and impact .
	manualset3
128252	5	405842	13	NULL	NULL	0	NULL	impact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	ROCK : the Roche medicinal chemistry knowledge application - design , use and impact .
	manualset3
128253	1	405843	13	NULL	NULL	0	NULL	ROS lipid	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	ROS lipid and fatty acid composition were not consistently different in dark and light groups .
	manualset3
128254	2	405843	13	NULL	NULL	NULL	NULL	fatty acid composition	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ROS lipid and fatty acid composition were not consistently different in dark and light groups .
	manualset3
128255	3	405843	13	NULL	NULL	0	NULL	dark groups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	ROS lipid and fatty acid composition were not consistently different in dark and light groups .
	manualset3
128256	4	405843	13	NULL	NULL	0	NULL	light groups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	ROS lipid and fatty acid composition were not consistently different in dark and light groups .
	manualset3
128257	1	405844	13	NULL	NULL	0	NULL	RPCI-24 mBESs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	RPCI-24 mBESs have more Q20 bases and longer reads on average than RPCI-23 sequences .
	manualset3
128258	2	405844	13	NULL	NULL	0	NULL	Q20 bases	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	RPCI-24 mBESs have more Q20 bases and longer reads on average than RPCI-23 sequences .
	manualset3
128259	3	405844	13	NULL	NULL	0	NULL	RPCI-23 sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	RPCI-24 mBESs have more Q20 bases and longer reads on average than RPCI-23 sequences .
	manualset3
128260	1	405845	13	NULL	NULL	0	NULL	RSV vaccine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	RSV vaccine development has been stifled for the past 23 years because infants vaccinated with formalin-inactivated ( FI ) RSV have experienced exacerbated disease upon RSV infection .
	manualset3
128261	2	405845	13	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	RSV vaccine development has been stifled for the past 23 years because infants vaccinated with formalin-inactivated ( FI ) RSV have experienced exacerbated disease upon RSV infection .
	manualset3
128262	3	405845	13	NULL	NULL	0	NULL	past 23 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	RSV vaccine development has been stifled for the past 23 years because infants vaccinated with formalin-inactivated ( FI ) RSV have experienced exacerbated disease upon RSV infection .
	manualset3
128263	4	405845	13	NULL	NULL	0	NULL	infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	RSV vaccine development has been stifled for the past 23 years because infants vaccinated with formalin-inactivated ( FI ) RSV have experienced exacerbated disease upon RSV infection .
	manualset3
128264	5	405845	13	NULL	NULL	0	NULL	formalin-inactivated ( FI ) RSV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	RSV vaccine development has been stifled for the past 23 years because infants vaccinated with formalin-inactivated ( FI ) RSV have experienced exacerbated disease upon RSV infection .
	manualset3
128265	6	405845	13	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	RSV vaccine development has been stifled for the past 23 years because infants vaccinated with formalin-inactivated ( FI ) RSV have experienced exacerbated disease upon RSV infection .
	manualset3
128266	7	405845	13	NULL	NULL	0	NULL	RSV infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	RSV vaccine development has been stifled for the past 23 years because infants vaccinated with formalin-inactivated ( FI ) RSV have experienced exacerbated disease upon RSV infection .
	manualset3
128267	1	405846	13	NULL	NULL	0	NULL	RT-PCR analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	RT-PCR analysis revealed similar levels of VEGFR-3 expression in all regions of the adult rat CNS .
	manualset3
128268	2	405846	13	NULL	NULL	0	NULL	levels 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	RT-PCR analysis revealed similar levels of VEGFR-3 expression in all regions of the adult rat CNS .
	manualset3
128269	3	405846	13	NULL	NULL	0	NULL	VEGFR-3 expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RT-PCR analysis revealed similar levels of VEGFR-3 expression in all regions of the adult rat CNS .
	manualset3
128270	4	405846	13	NULL	NULL	0	NULL	regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	RT-PCR analysis revealed similar levels of VEGFR-3 expression in all regions of the adult rat CNS .
	manualset3
128271	5	405846	13	NULL	NULL	0	NULL	adult rat CNS	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	RT-PCR analysis revealed similar levels of VEGFR-3 expression in all regions of the adult rat CNS .
	manualset3
128272	1	405847	13	NULL	NULL	0	NULL	RT-PCR assay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	RT-PCR assay was performed to detect the expression of miR-21 in 10 pairs of OSCC and noncancerous tissue samples .
	manualset3
128273	2	405847	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RT-PCR assay was performed to detect the expression of miR-21 in 10 pairs of OSCC and noncancerous tissue samples .
	manualset3
128274	3	405847	13	NULL	NULL	0	NULL	miR-21	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	RT-PCR assay was performed to detect the expression of miR-21 in 10 pairs of OSCC and noncancerous tissue samples .
	manualset3
128275	4	405847	13	NULL	NULL	0	NULL	10 pairs	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	RT-PCR assay was performed to detect the expression of miR-21 in 10 pairs of OSCC and noncancerous tissue samples .
	manualset3
128276	5	405847	13	NULL	NULL	0	NULL	OSCC samples	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	RT-PCR assay was performed to detect the expression of miR-21 in 10 pairs of OSCC and noncancerous tissue samples .
	manualset3
128277	6	405847	13	NULL	NULL	0	NULL	noncancerous tissue samples	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	RT-PCR assay was performed to detect the expression of miR-21 in 10 pairs of OSCC and noncancerous tissue samples .
	manualset3
128278	1	405848	13	NULL	NULL	0	NULL	RU 24969	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	RU 24969 significantly reduced Bmax 23 to 63 % in cortex , hippocampus , striatum , brainstem , and spinal cord without a change in Ka except for a 1.7-fold increase in cortex and spinal cord .
	manualset3
128279	2	405848	13	NULL	NULL	0	NULL	Bmax	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	RU 24969 significantly reduced Bmax 23 to 63 % in cortex , hippocampus , striatum , brainstem , and spinal cord without a change in Ka except for a 1.7-fold increase in cortex and spinal cord .
	manualset3
128280	3	405848	13	NULL	NULL	0	NULL	23 to 63 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	RU 24969 significantly reduced Bmax 23 to 63 % in cortex , hippocampus , striatum , brainstem , and spinal cord without a change in Ka except for a 1.7-fold increase in cortex and spinal cord .
	manualset3
128281	4	405848	13	NULL	NULL	0	NULL	cortex 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	RU 24969 significantly reduced Bmax 23 to 63 % in cortex , hippocampus , striatum , brainstem , and spinal cord without a change in Ka except for a 1.7-fold increase in cortex and spinal cord .
	manualset3
128282	5	405848	13	NULL	NULL	0	NULL	hippocampus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	RU 24969 significantly reduced Bmax 23 to 63 % in cortex , hippocampus , striatum , brainstem , and spinal cord without a change in Ka except for a 1.7-fold increase in cortex and spinal cord .
	manualset3
128283	6	405848	13	NULL	NULL	0	NULL	striatum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	RU 24969 significantly reduced Bmax 23 to 63 % in cortex , hippocampus , striatum , brainstem , and spinal cord without a change in Ka except for a 1.7-fold increase in cortex and spinal cord .
	manualset3
128284	7	405848	13	NULL	NULL	0	NULL	brainstem	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	RU 24969 significantly reduced Bmax 23 to 63 % in cortex , hippocampus , striatum , brainstem , and spinal cord without a change in Ka except for a 1.7-fold increase in cortex and spinal cord .
	manualset3
128285	8	405848	13	NULL	NULL	0	NULL	spinal cord	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	RU 24969 significantly reduced Bmax 23 to 63 % in cortex , hippocampus , striatum , brainstem , and spinal cord without a change in Ka except for a 1.7-fold increase in cortex and spinal cord .
	manualset3
128286	9	405848	13	NULL	NULL	0	NULL	change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	RU 24969 significantly reduced Bmax 23 to 63 % in cortex , hippocampus , striatum , brainstem , and spinal cord without a change in Ka except for a 1.7-fold increase in cortex and spinal cord .
	manualset3
128287	10	405848	13	NULL	NULL	0	NULL	Ka	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	RU 24969 significantly reduced Bmax 23 to 63 % in cortex , hippocampus , striatum , brainstem , and spinal cord without a change in Ka except for a 1.7-fold increase in cortex and spinal cord .
	manualset3
128288	11	405848	13	NULL	NULL	NULL	NULL	1.7-fold	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	RU 24969 significantly reduced Bmax 23 to 63 % in cortex , hippocampus , striatum , brainstem , and spinal cord without a change in Ka except for a 1.7-fold increase in cortex and spinal cord .
	manualset3
128289	12	405848	13	NULL	NULL	0	NULL	cortex 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	RU 24969 significantly reduced Bmax 23 to 63 % in cortex , hippocampus , striatum , brainstem , and spinal cord without a change in Ka except for a 1.7-fold increase in cortex and spinal cord .
	manualset3
128290	13	405848	13	NULL	NULL	0	NULL	spinal cord 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	RU 24969 significantly reduced Bmax 23 to 63 % in cortex , hippocampus , striatum , brainstem , and spinal cord without a change in Ka except for a 1.7-fold increase in cortex and spinal cord .
	manualset3
128291	1	405849	13	NULL	NULL	0	NULL	Rabbit skeletal muscle myosin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Rabbit skeletal muscle myosin , in the presence of rabbit skeletal troponin : tropomyosin , also shows full apparent activation by free lanthanide .
	manualset3
128292	2	405849	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rabbit skeletal muscle myosin , in the presence of rabbit skeletal troponin : tropomyosin , also shows full apparent activation by free lanthanide .
	manualset3
128293	3	405849	13	NULL	NULL	0	NULL	 rabbit skeletal troponin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Rabbit skeletal muscle myosin , in the presence of rabbit skeletal troponin : tropomyosin , also shows full apparent activation by free lanthanide .
	manualset3
128294	4	405849	13	NULL	NULL	0	NULL	tropomyosin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Rabbit skeletal muscle myosin , in the presence of rabbit skeletal troponin : tropomyosin , also shows full apparent activation by free lanthanide .
	manualset3
128295	5	405849	13	NULL	NULL	0	NULL	activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rabbit skeletal muscle myosin , in the presence of rabbit skeletal troponin : tropomyosin , also shows full apparent activation by free lanthanide .
	manualset3
128296	6	405849	13	NULL	NULL	0	NULL	free lanthanide	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Rabbit skeletal muscle myosin , in the presence of rabbit skeletal troponin : tropomyosin , also shows full apparent activation by free lanthanide .
	manualset3
128297	1	405850	13	NULL	NULL	0	NULL	Rabies encephalitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Rabies encephalitis still generates 50 , 000 human deaths/year .
	manualset3
128298	2	405850	13	NULL	NULL	0	NULL	50 , 000 human deaths/year 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rabies encephalitis still generates 50 , 000 human deaths/year .
	manualset3
128299	1	405851	13	NULL	NULL	0	NULL	Racial centrality	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Racial centrality related positively to school performance and school importance attitudes for boys .
	manualset3
128300	2	405851	13	NULL	NULL	0	NULL	school performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Racial centrality related positively to school performance and school importance attitudes for boys .
	manualset3
128301	3	405851	13	NULL	NULL	0	NULL	school importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Racial centrality related positively to school performance and school importance attitudes for boys .
	manualset3
128302	4	405851	13	NULL	NULL	0	NULL	attitudes 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Racial centrality related positively to school performance and school importance attitudes for boys .
	manualset3
128303	5	405851	13	NULL	NULL	0	NULL	boys	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Racial centrality related positively to school performance and school importance attitudes for boys .
	manualset3
128304	1	405852	13	NULL	NULL	NULL	NULL	Radiation Resistance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Radiation Resistance in Cancer Therapy : meeting summary and research opportunities .
	manualset3
128305	2	405852	13	NULL	NULL	0	NULL	Cancer Therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation Resistance in Cancer Therapy : meeting summary and research opportunities .
	manualset3
128306	3	405852	13	NULL	NULL	0	NULL	meeting summary 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation Resistance in Cancer Therapy : meeting summary and research opportunities .
	manualset3
128307	4	405852	13	NULL	NULL	0	NULL	research opportunities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation Resistance in Cancer Therapy : meeting summary and research opportunities .
	manualset3
128308	1	405853	13	NULL	NULL	0	NULL	Radiation distributions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation distributions produced by both sealed sources commonly used in brachytherapy ( 192I , 137Cs , 226Ra ) and an unsealed source used in the treatment of the thyroid ( 131I ) were used to irradiate a Rando phantom .
	manualset3
128309	2	405853	13	NULL	NULL	0	NULL	sources	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation distributions produced by both sealed sources commonly used in brachytherapy ( 192I , 137Cs , 226Ra ) and an unsealed source used in the treatment of the thyroid ( 131I ) were used to irradiate a Rando phantom .
	manualset3
128310	3	405853	13	NULL	NULL	0	NULL	brachytherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation distributions produced by both sealed sources commonly used in brachytherapy ( 192I , 137Cs , 226Ra ) and an unsealed source used in the treatment of the thyroid ( 131I ) were used to irradiate a Rando phantom .
	manualset3
128311	4	405853	13	NULL	NULL	0	NULL	192I	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation distributions produced by both sealed sources commonly used in brachytherapy ( 192I , 137Cs , 226Ra ) and an unsealed source used in the treatment of the thyroid ( 131I ) were used to irradiate a Rando phantom .
	manualset3
128312	5	405853	13	NULL	NULL	0	NULL	137Cs	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation distributions produced by both sealed sources commonly used in brachytherapy ( 192I , 137Cs , 226Ra ) and an unsealed source used in the treatment of the thyroid ( 131I ) were used to irradiate a Rando phantom .
	manualset3
128313	6	405853	13	NULL	NULL	0	NULL	226Ra	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation distributions produced by both sealed sources commonly used in brachytherapy ( 192I , 137Cs , 226Ra ) and an unsealed source used in the treatment of the thyroid ( 131I ) were used to irradiate a Rando phantom .
	manualset3
128314	7	405853	13	NULL	NULL	0	NULL	source	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation distributions produced by both sealed sources commonly used in brachytherapy ( 192I , 137Cs , 226Ra ) and an unsealed source used in the treatment of the thyroid ( 131I ) were used to irradiate a Rando phantom .
	manualset3
128315	8	405853	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation distributions produced by both sealed sources commonly used in brachytherapy ( 192I , 137Cs , 226Ra ) and an unsealed source used in the treatment of the thyroid ( 131I ) were used to irradiate a Rando phantom .
	manualset3
128316	9	405853	13	NULL	NULL	NULL	NULL	thyroid 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Radiation distributions produced by both sealed sources commonly used in brachytherapy ( 192I , 137Cs , 226Ra ) and an unsealed source used in the treatment of the thyroid ( 131I ) were used to irradiate a Rando phantom .
	manualset3
128317	10	405853	13	NULL	NULL	0	NULL	Rando phantom	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation distributions produced by both sealed sources commonly used in brachytherapy ( 192I , 137Cs , 226Ra ) and an unsealed source used in the treatment of the thyroid ( 131I ) were used to irradiate a Rando phantom .
	manualset3
129238	11	405853	13	NULL	NULL	0	NULL	131I	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation distributions produced by both sealed sources commonly used in brachytherapy ( 192I , 137Cs , 226Ra ) and an unsealed source used in the treatment of the thyroid ( 131I ) were used to irradiate a Rando phantom .
	manualset3
128318	1	405854	13	NULL	NULL	0	NULL	Radiation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation induced bowel damage affects 6000 individuals annually in the UK , with a negative impact on quality of life .
	manualset3
128319	2	405854	13	NULL	NULL	0	NULL	bowel damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation induced bowel damage affects 6000 individuals annually in the UK , with a negative impact on quality of life .
	manualset3
128320	3	405854	13	NULL	NULL	0	NULL	6000 individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation induced bowel damage affects 6000 individuals annually in the UK , with a negative impact on quality of life .
	manualset3
128321	4	405854	13	NULL	NULL	0	NULL	UK 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation induced bowel damage affects 6000 individuals annually in the UK , with a negative impact on quality of life .
	manualset3
128322	5	405854	13	NULL	NULL	0	NULL	negative impact	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation induced bowel damage affects 6000 individuals annually in the UK , with a negative impact on quality of life .
	manualset3
128323	6	405854	13	NULL	NULL	0	NULL	quality of life	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation induced bowel damage affects 6000 individuals annually in the UK , with a negative impact on quality of life .
	manualset3
128324	1	405855	13	NULL	NULL	0	NULL	Radiation oncologist	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation oncologist , pulmonologists and thoracic surgeons are assiduous to these meeting ; however radiologists and , to a lesser extent , pathologists are less attentive .
	manualset3
128325	2	405855	13	NULL	NULL	0	NULL	pulmonologists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation oncologist , pulmonologists and thoracic surgeons are assiduous to these meeting ; however radiologists and , to a lesser extent , pathologists are less attentive .
	manualset3
128326	3	405855	13	NULL	NULL	0	NULL	thoracic surgeons 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation oncologist , pulmonologists and thoracic surgeons are assiduous to these meeting ; however radiologists and , to a lesser extent , pathologists are less attentive .
	manualset3
128327	4	405855	13	NULL	NULL	0	NULL	meeting 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation oncologist , pulmonologists and thoracic surgeons are assiduous to these meeting ; however radiologists and , to a lesser extent , pathologists are less attentive .
	manualset3
128328	5	405855	13	NULL	NULL	0	NULL	radiologists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation oncologist , pulmonologists and thoracic surgeons are assiduous to these meeting ; however radiologists and , to a lesser extent , pathologists are less attentive .
	manualset3
128329	6	405855	13	NULL	NULL	0	NULL	extent	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation oncologist , pulmonologists and thoracic surgeons are assiduous to these meeting ; however radiologists and , to a lesser extent , pathologists are less attentive .
	manualset3
128330	7	405855	13	NULL	NULL	0	NULL	pathologists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation oncologist , pulmonologists and thoracic surgeons are assiduous to these meeting ; however radiologists and , to a lesser extent , pathologists are less attentive .
	manualset3
128331	1	405856	13	NULL	NULL	0	NULL	Radiation therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation therapy after R-CHOP for diffuse large B-cell lymphoma : the gain remains .
	manualset3
128332	2	405856	13	NULL	NULL	0	NULL	R-CHOP	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation therapy after R-CHOP for diffuse large B-cell lymphoma : the gain remains .
	manualset3
128333	3	405856	13	NULL	NULL	0	NULL	diffuse large B-cell lymphoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation therapy after R-CHOP for diffuse large B-cell lymphoma : the gain remains .
	manualset3
128334	4	405856	13	NULL	NULL	0	NULL	gain	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation therapy after R-CHOP for diffuse large B-cell lymphoma : the gain remains .
	manualset3
128335	1	405857	13	NULL	NULL	0	NULL	Radiation therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation therapy is the mainstay of treatment while surgery or chemotherapy is used in selected patients .
	manualset3
128336	2	405857	13	NULL	NULL	0	NULL	mainstay	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation therapy is the mainstay of treatment while surgery or chemotherapy is used in selected patients .
	manualset3
128337	3	405857	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation therapy is the mainstay of treatment while surgery or chemotherapy is used in selected patients .
	manualset3
128338	4	405857	13	NULL	NULL	0	NULL	surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation therapy is the mainstay of treatment while surgery or chemotherapy is used in selected patients .
	manualset3
128339	5	405857	13	NULL	NULL	0	NULL	chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation therapy is the mainstay of treatment while surgery or chemotherapy is used in selected patients .
	manualset3
128340	6	405857	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation therapy is the mainstay of treatment while surgery or chemotherapy is used in selected patients .
	manualset3
128341	1	405858	13	NULL	NULL	0	NULL	membrane oxygen electrode	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A membrane oxygen electrode usually suffers from long-term signal deterioration due to environmental factors such as changes in hydrodynamic conditions and alteration of membrane oxygen diffusivity due to fouling .
	manualset3
128342	2	405858	13	NULL	NULL	0	NULL	long-term signal deterioration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A membrane oxygen electrode usually suffers from long-term signal deterioration due to environmental factors such as changes in hydrodynamic conditions and alteration of membrane oxygen diffusivity due to fouling .
	manualset3
128343	3	405858	13	NULL	NULL	0	NULL	environmental factors	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A membrane oxygen electrode usually suffers from long-term signal deterioration due to environmental factors such as changes in hydrodynamic conditions and alteration of membrane oxygen diffusivity due to fouling .
	manualset3
128344	4	405858	13	NULL	NULL	0	NULL	changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A membrane oxygen electrode usually suffers from long-term signal deterioration due to environmental factors such as changes in hydrodynamic conditions and alteration of membrane oxygen diffusivity due to fouling .
	manualset3
128345	5	405858	13	NULL	NULL	0	NULL	hydrodynamic conditions 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A membrane oxygen electrode usually suffers from long-term signal deterioration due to environmental factors such as changes in hydrodynamic conditions and alteration of membrane oxygen diffusivity due to fouling .
	manualset3
128346	6	405858	13	NULL	NULL	0	NULL	 alteration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A membrane oxygen electrode usually suffers from long-term signal deterioration due to environmental factors such as changes in hydrodynamic conditions and alteration of membrane oxygen diffusivity due to fouling .
	manualset3
128347	7	405858	13	NULL	NULL	NULL	NULL	membrane oxygen diffusivity	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A membrane oxygen electrode usually suffers from long-term signal deterioration due to environmental factors such as changes in hydrodynamic conditions and alteration of membrane oxygen diffusivity due to fouling .
	manualset3
128348	8	405858	13	NULL	NULL	0	NULL	fouling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A membrane oxygen electrode usually suffers from long-term signal deterioration due to environmental factors such as changes in hydrodynamic conditions and alteration of membrane oxygen diffusivity due to fouling .
	manualset3
128349	1	405859	13	NULL	NULL	0	NULL	Radiation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation was delivered from TOC-1001 neodymium laser , wave-length of 1 , 060 nm , pulse duration -- 1 msec and fluence -- 350-400 J/cm2 .
	manualset3
128350	2	405859	13	NULL	NULL	0	NULL	TOC-1001 neodymium laser	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation was delivered from TOC-1001 neodymium laser , wave-length of 1 , 060 nm , pulse duration -- 1 msec and fluence -- 350-400 J/cm2 .
	manualset3
128351	3	405859	13	NULL	NULL	0	NULL	wave-length of 1 , 060 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation was delivered from TOC-1001 neodymium laser , wave-length of 1 , 060 nm , pulse duration -- 1 msec and fluence -- 350-400 J/cm2 .
	manualset3
128352	4	405859	13	NULL	NULL	NULL	NULL	pulse duration -- 1 msec 	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Radiation was delivered from TOC-1001 neodymium laser , wave-length of 1 , 060 nm , pulse duration -- 1 msec and fluence -- 350-400 J/cm2 .
	manualset3
128353	5	405859	13	NULL	NULL	0	NULL	fluence -- 350-400 J/cm2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiation was delivered from TOC-1001 neodymium laser , wave-length of 1 , 060 nm , pulse duration -- 1 msec and fluence -- 350-400 J/cm2 .
	manualset3
128354	1	405860	13	NULL	NULL	0	NULL	Radical resection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Radical resection for the treatment of glioma .
	manualset3
128355	2	405860	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Radical resection for the treatment of glioma .
	manualset3
128356	3	405860	13	NULL	NULL	NULL	NULL	glioma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Radical resection for the treatment of glioma .
	manualset3
128357	1	405861	13	NULL	NULL	0	NULL	methionine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioactively labeled methionine , leucine , glycine , serine , beta-alanine and taurine ( concentrations less than or equal to 5 microM ) were also taken up by ganglia .
	manualset3
128358	2	405861	13	NULL	NULL	0	NULL	leucine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioactively labeled methionine , leucine , glycine , serine , beta-alanine and taurine ( concentrations less than or equal to 5 microM ) were also taken up by ganglia .
	manualset3
128359	3	405861	13	NULL	NULL	0	NULL	glycine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioactively labeled methionine , leucine , glycine , serine , beta-alanine and taurine ( concentrations less than or equal to 5 microM ) were also taken up by ganglia .
	manualset3
128360	4	405861	13	NULL	NULL	0	NULL	serine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioactively labeled methionine , leucine , glycine , serine , beta-alanine and taurine ( concentrations less than or equal to 5 microM ) were also taken up by ganglia .
	manualset3
128361	5	405861	13	NULL	NULL	0	NULL	beta-alanine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioactively labeled methionine , leucine , glycine , serine , beta-alanine and taurine ( concentrations less than or equal to 5 microM ) were also taken up by ganglia .
	manualset3
128362	6	405861	13	NULL	NULL	0	NULL	taurine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioactively labeled methionine , leucine , glycine , serine , beta-alanine and taurine ( concentrations less than or equal to 5 microM ) were also taken up by ganglia .
	manualset3
128363	7	405861	13	NULL	NULL	0	NULL	concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioactively labeled methionine , leucine , glycine , serine , beta-alanine and taurine ( concentrations less than or equal to 5 microM ) were also taken up by ganglia .
	manualset3
128364	8	405861	13	NULL	NULL	0	NULL	5 microM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioactively labeled methionine , leucine , glycine , serine , beta-alanine and taurine ( concentrations less than or equal to 5 microM ) were also taken up by ganglia .
	manualset3
128365	9	405861	13	NULL	NULL	0	NULL	ganglia	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioactively labeled methionine , leucine , glycine , serine , beta-alanine and taurine ( concentrations less than or equal to 5 microM ) were also taken up by ganglia .
	manualset3
128366	1	405862	13	NULL	NULL	0	NULL	Radioautography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioautography with tritiated thymidine indicated a constant cell renewal in epithelium and monolayer apparently from foci of p-cells , a reserve population of which was seen to be sequestered among the smooth muscle cells .
	manualset3
128367	2	405862	13	NULL	NULL	0	NULL	thymidine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioautography with tritiated thymidine indicated a constant cell renewal in epithelium and monolayer apparently from foci of p-cells , a reserve population of which was seen to be sequestered among the smooth muscle cells .
	manualset3
128368	3	405862	13	NULL	NULL	0	NULL	cell renewal	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioautography with tritiated thymidine indicated a constant cell renewal in epithelium and monolayer apparently from foci of p-cells , a reserve population of which was seen to be sequestered among the smooth muscle cells .
	manualset3
128369	4	405862	13	NULL	NULL	0	NULL	epithelium	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioautography with tritiated thymidine indicated a constant cell renewal in epithelium and monolayer apparently from foci of p-cells , a reserve population of which was seen to be sequestered among the smooth muscle cells .
	manualset3
128370	5	405862	13	NULL	NULL	0	NULL	monolayer 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioautography with tritiated thymidine indicated a constant cell renewal in epithelium and monolayer apparently from foci of p-cells , a reserve population of which was seen to be sequestered among the smooth muscle cells .
	manualset3
128371	6	405862	13	NULL	NULL	0	NULL	foci of p-cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioautography with tritiated thymidine indicated a constant cell renewal in epithelium and monolayer apparently from foci of p-cells , a reserve population of which was seen to be sequestered among the smooth muscle cells .
	manualset3
128372	7	405862	13	NULL	NULL	0	NULL	population	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioautography with tritiated thymidine indicated a constant cell renewal in epithelium and monolayer apparently from foci of p-cells , a reserve population of which was seen to be sequestered among the smooth muscle cells .
	manualset3
128373	8	405862	13	NULL	NULL	0	NULL	smooth muscle cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioautography with tritiated thymidine indicated a constant cell renewal in epithelium and monolayer apparently from foci of p-cells , a reserve population of which was seen to be sequestered among the smooth muscle cells .
	manualset3
128374	1	405863	13	NULL	NULL	0	NULL	Radiocesium levels 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiocesium levels were strongly dependent on the duration of residence in Israel , with the highest levels being found in the most recent immigrants .
	manualset3
128375	2	405863	13	NULL	NULL	0	NULL	duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiocesium levels were strongly dependent on the duration of residence in Israel , with the highest levels being found in the most recent immigrants .
	manualset3
128376	3	405863	13	NULL	NULL	0	NULL	residence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiocesium levels were strongly dependent on the duration of residence in Israel , with the highest levels being found in the most recent immigrants .
	manualset3
128377	4	405863	13	NULL	NULL	0	NULL	Israel	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiocesium levels were strongly dependent on the duration of residence in Israel , with the highest levels being found in the most recent immigrants .
	manualset3
128378	5	405863	13	NULL	NULL	0	NULL	levels 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiocesium levels were strongly dependent on the duration of residence in Israel , with the highest levels being found in the most recent immigrants .
	manualset3
128379	6	405863	13	NULL	NULL	0	NULL	immigrants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiocesium levels were strongly dependent on the duration of residence in Israel , with the highest levels being found in the most recent immigrants .
	manualset3
128380	1	405864	13	NULL	NULL	0	NULL	Radiochemical analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiochemical and chemical analysis of the carbohydrate moieties of two myeloma proteins purified from different subcellular fractions of plasma cells .
	manualset3
128381	2	405864	13	NULL	NULL	0	NULL	carbohydrate moieties	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiochemical and chemical analysis of the carbohydrate moieties of two myeloma proteins purified from different subcellular fractions of plasma cells .
	manualset3
128382	3	405864	13	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiochemical and chemical analysis of the carbohydrate moieties of two myeloma proteins purified from different subcellular fractions of plasma cells .
	manualset3
128383	4	405864	13	NULL	NULL	0	NULL	myeloma proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiochemical and chemical analysis of the carbohydrate moieties of two myeloma proteins purified from different subcellular fractions of plasma cells .
	manualset3
128384	5	405864	13	NULL	NULL	0	NULL	subcellular fractions	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiochemical and chemical analysis of the carbohydrate moieties of two myeloma proteins purified from different subcellular fractions of plasma cells .
	manualset3
128385	6	405864	13	NULL	NULL	0	NULL	plasma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiochemical and chemical analysis of the carbohydrate moieties of two myeloma proteins purified from different subcellular fractions of plasma cells .
	manualset3
128386	7	405864	13	NULL	NULL	0	NULL	chemical analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiochemical and chemical analysis of the carbohydrate moieties of two myeloma proteins purified from different subcellular fractions of plasma cells .
	manualset3
128387	1	405865	13	NULL	NULL	0	NULL	Radiocontrast nephropathy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiocontrast nephropathy is associated with increased morbidity , prolonged hospitalization , and higher in-hospital mortality .
	manualset3
128388	2	405865	13	NULL	NULL	0	NULL	morbidity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiocontrast nephropathy is associated with increased morbidity , prolonged hospitalization , and higher in-hospital mortality .
	manualset3
128389	3	405865	13	NULL	NULL	0	NULL	hospitalization 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiocontrast nephropathy is associated with increased morbidity , prolonged hospitalization , and higher in-hospital mortality .
	manualset3
128390	4	405865	13	NULL	NULL	0	NULL	in-hospital mortality 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiocontrast nephropathy is associated with increased morbidity , prolonged hospitalization , and higher in-hospital mortality .
	manualset3
128391	1	405866	13	NULL	NULL	0	NULL	Radiographic abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiographic abnormalities include indentations of vertebral outline and radiolucencies within the vertebral body with varying degrees of sclerosis .
	manualset3
128392	2	405866	13	NULL	NULL	0	NULL	indentations 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiographic abnormalities include indentations of vertebral outline and radiolucencies within the vertebral body with varying degrees of sclerosis .
	manualset3
128393	3	405866	13	NULL	NULL	0	NULL	vertebral outline 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiographic abnormalities include indentations of vertebral outline and radiolucencies within the vertebral body with varying degrees of sclerosis .
	manualset3
128394	4	405866	13	NULL	NULL	0	NULL	radiolucencies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiographic abnormalities include indentations of vertebral outline and radiolucencies within the vertebral body with varying degrees of sclerosis .
	manualset3
128395	5	405866	13	NULL	NULL	0	NULL	vertebral body 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiographic abnormalities include indentations of vertebral outline and radiolucencies within the vertebral body with varying degrees of sclerosis .
	manualset3
128396	6	405866	13	NULL	NULL	0	NULL	degrees of sclerosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiographic abnormalities include indentations of vertebral outline and radiolucencies within the vertebral body with varying degrees of sclerosis .
	manualset3
128397	1	405867	13	NULL	NULL	0	NULL	memory-training program	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A memory-training program previously used effectively upon persons with head-injury ( HI ) was conducted upon eight subjects with multiple sclerosis ( MS ) .
	manualset3
128398	2	405867	13	NULL	NULL	0	NULL	persons 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A memory-training program previously used effectively upon persons with head-injury ( HI ) was conducted upon eight subjects with multiple sclerosis ( MS ) .
	manualset3
128399	3	405867	13	NULL	NULL	0	NULL	head-injury ( HI ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A memory-training program previously used effectively upon persons with head-injury ( HI ) was conducted upon eight subjects with multiple sclerosis ( MS ) .
	manualset3
128400	4	405867	13	NULL	NULL	0	NULL	eight subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A memory-training program previously used effectively upon persons with head-injury ( HI ) was conducted upon eight subjects with multiple sclerosis ( MS ) .
	manualset3
128401	5	405867	13	NULL	NULL	0	NULL	multiple sclerosis ( MS ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A memory-training program previously used effectively upon persons with head-injury ( HI ) was conducted upon eight subjects with multiple sclerosis ( MS ) .
	manualset3
128402	1	405868	13	NULL	NULL	NULL	NULL	Radiographic techniques	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Radiographic techniques , such as computerised tomography and ultrasonography , as well as magnetic resonance imaging , are used widely for confirmation and follow-up of the disease .
	manualset3
128403	2	405868	13	NULL	NULL	NULL	NULL	computerised tomography	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Radiographic techniques , such as computerised tomography and ultrasonography , as well as magnetic resonance imaging , are used widely for confirmation and follow-up of the disease .
	manualset3
128404	3	405868	13	NULL	NULL	0	NULL	ultrasonography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiographic techniques , such as computerised tomography and ultrasonography , as well as magnetic resonance imaging , are used widely for confirmation and follow-up of the disease .
	manualset3
128405	4	405868	13	NULL	NULL	0	NULL	magnetic resonance imaging 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiographic techniques , such as computerised tomography and ultrasonography , as well as magnetic resonance imaging , are used widely for confirmation and follow-up of the disease .
	manualset3
128406	5	405868	13	NULL	NULL	0	NULL	confirmation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiographic techniques , such as computerised tomography and ultrasonography , as well as magnetic resonance imaging , are used widely for confirmation and follow-up of the disease .
	manualset3
128407	6	405868	13	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiographic techniques , such as computerised tomography and ultrasonography , as well as magnetic resonance imaging , are used widely for confirmation and follow-up of the disease .
	manualset3
131915	7	405868	13	NULL	NULL	0	NULL	follow-up	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiographic techniques , such as computerised tomography and ultrasonography , as well as magnetic resonance imaging , are used widely for confirmation and follow-up of the disease .
	manualset3
128408	1	405869	13	NULL	NULL	0	NULL	Radiographs	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiographs revealed no failures of ingrowth at last follow-up .
	manualset3
128409	2	405869	13	NULL	NULL	0	NULL	failures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiographs revealed no failures of ingrowth at last follow-up .
	manualset3
128410	3	405869	13	NULL	NULL	0	NULL	 ingrowth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiographs revealed no failures of ingrowth at last follow-up .
	manualset3
128411	4	405869	13	NULL	NULL	0	NULL	follow-up	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiographs revealed no failures of ingrowth at last follow-up .
	manualset3
128412	1	405870	13	NULL	NULL	0	NULL	Radioimmunoassays 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioimmunoassays were used to measure the non-adrenergic , non-cholinergic inhibitory neuropeptide , vasoactive intestinal peptide , and the non-adrenergic , non-cholinergic excitatory neuropeptide , substance P , while spectrophotometric assays were used to quantitate acetylcholinesterase activity and choline acetyltransferase activity .
	manualset3
128413	2	405870	13	NULL	NULL	0	NULL	non-adrenergic inhibitory neuropeptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioimmunoassays were used to measure the non-adrenergic , non-cholinergic inhibitory neuropeptide , vasoactive intestinal peptide , and the non-adrenergic , non-cholinergic excitatory neuropeptide , substance P , while spectrophotometric assays were used to quantitate acetylcholinesterase activity and choline acetyltransferase activity .
	manualset3
128414	3	405870	13	NULL	NULL	0	NULL	non-cholinergic inhibitory neuropeptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioimmunoassays were used to measure the non-adrenergic , non-cholinergic inhibitory neuropeptide , vasoactive intestinal peptide , and the non-adrenergic , non-cholinergic excitatory neuropeptide , substance P , while spectrophotometric assays were used to quantitate acetylcholinesterase activity and choline acetyltransferase activity .
	manualset3
128415	4	405870	13	NULL	NULL	0	NULL	vasoactive intestinal peptide 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioimmunoassays were used to measure the non-adrenergic , non-cholinergic inhibitory neuropeptide , vasoactive intestinal peptide , and the non-adrenergic , non-cholinergic excitatory neuropeptide , substance P , while spectrophotometric assays were used to quantitate acetylcholinesterase activity and choline acetyltransferase activity .
	manualset3
128416	5	405870	13	NULL	NULL	0	NULL	non-adrenergic excitatory neuropeptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioimmunoassays were used to measure the non-adrenergic , non-cholinergic inhibitory neuropeptide , vasoactive intestinal peptide , and the non-adrenergic , non-cholinergic excitatory neuropeptide , substance P , while spectrophotometric assays were used to quantitate acetylcholinesterase activity and choline acetyltransferase activity .
	manualset3
128417	6	405870	13	NULL	NULL	0	NULL	substance P 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioimmunoassays were used to measure the non-adrenergic , non-cholinergic inhibitory neuropeptide , vasoactive intestinal peptide , and the non-adrenergic , non-cholinergic excitatory neuropeptide , substance P , while spectrophotometric assays were used to quantitate acetylcholinesterase activity and choline acetyltransferase activity .
	manualset3
128418	7	405870	13	NULL	NULL	0	NULL	spectrophotometric assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioimmunoassays were used to measure the non-adrenergic , non-cholinergic inhibitory neuropeptide , vasoactive intestinal peptide , and the non-adrenergic , non-cholinergic excitatory neuropeptide , substance P , while spectrophotometric assays were used to quantitate acetylcholinesterase activity and choline acetyltransferase activity .
	manualset3
128419	8	405870	13	NULL	NULL	0	NULL	acetylcholinesterase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioimmunoassays were used to measure the non-adrenergic , non-cholinergic inhibitory neuropeptide , vasoactive intestinal peptide , and the non-adrenergic , non-cholinergic excitatory neuropeptide , substance P , while spectrophotometric assays were used to quantitate acetylcholinesterase activity and choline acetyltransferase activity .
	manualset3
128420	9	405870	13	NULL	NULL	0	NULL	choline acetyltransferase activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioimmunoassays were used to measure the non-adrenergic , non-cholinergic inhibitory neuropeptide , vasoactive intestinal peptide , and the non-adrenergic , non-cholinergic excitatory neuropeptide , substance P , while spectrophotometric assays were used to quantitate acetylcholinesterase activity and choline acetyltransferase activity .
	manualset3
128421	1	405871	13	NULL	NULL	0	NULL	Radioisotope scanning 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioisotope scanning and celiac angiography demonstrated lymphangiomatosis of the spleen , a rare but diagnosable condition .
	manualset3
128422	2	405871	13	NULL	NULL	0	NULL	celiac angiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioisotope scanning and celiac angiography demonstrated lymphangiomatosis of the spleen , a rare but diagnosable condition .
	manualset3
128423	3	405871	13	NULL	NULL	0	NULL	lymphangiomatosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioisotope scanning and celiac angiography demonstrated lymphangiomatosis of the spleen , a rare but diagnosable condition .
	manualset3
128424	4	405871	13	NULL	NULL	0	NULL	spleen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioisotope scanning and celiac angiography demonstrated lymphangiomatosis of the spleen , a rare but diagnosable condition .
	manualset3
128425	5	405871	13	NULL	NULL	0	NULL	diagnosable condition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioisotope scanning and celiac angiography demonstrated lymphangiomatosis of the spleen , a rare but diagnosable condition .
	manualset3
128426	1	405872	13	NULL	NULL	0	NULL	Radioisotopic evaluation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioisotopic evaluation of renal parenchymal disorders in children .
	manualset3
128427	2	405872	13	NULL	NULL	0	NULL	renal parenchymal disorders 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioisotopic evaluation of renal parenchymal disorders in children .
	manualset3
128428	3	405872	13	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioisotopic evaluation of renal parenchymal disorders in children .
	manualset3
128429	1	405873	13	NULL	NULL	0	NULL	Radiolabeled steroids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiolabeled steroids were directly perfused in the dextran-blood into either the left or right half of the hypothalamus .
	manualset3
128430	2	405873	13	NULL	NULL	0	NULL	dextran-blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiolabeled steroids were directly perfused in the dextran-blood into either the left or right half of the hypothalamus .
	manualset3
128431	3	405873	13	NULL	NULL	0	NULL	left half of the hypothalamus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiolabeled steroids were directly perfused in the dextran-blood into either the left or right half of the hypothalamus .
	manualset3
128432	4	405873	13	NULL	NULL	0	NULL	right half of the hypothalamus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiolabeled steroids were directly perfused in the dextran-blood into either the left or right half of the hypothalamus .
	manualset3
128433	1	405874	13	NULL	NULL	0	NULL	piperidine derivatives 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiolabelled piperidine derivatives such as ( ( 11 ) C ) MDL 100907 and ( ( 18 ) F ) altanserin have played an important role in diagnosing malfunction in the serotonergic neurotransmission .
	manualset3
128434	2	405874	13	NULL	NULL	0	NULL	( ( 11 ) C ) MDL 100907 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiolabelled piperidine derivatives such as ( ( 11 ) C ) MDL 100907 and ( ( 18 ) F ) altanserin have played an important role in diagnosing malfunction in the serotonergic neurotransmission .
	manualset3
128435	3	405874	13	NULL	NULL	0	NULL	( ( 18 ) F ) altanserin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiolabelled piperidine derivatives such as ( ( 11 ) C ) MDL 100907 and ( ( 18 ) F ) altanserin have played an important role in diagnosing malfunction in the serotonergic neurotransmission .
	manualset3
128436	4	405874	13	NULL	NULL	0	NULL	role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiolabelled piperidine derivatives such as ( ( 11 ) C ) MDL 100907 and ( ( 18 ) F ) altanserin have played an important role in diagnosing malfunction in the serotonergic neurotransmission .
	manualset3
128437	5	405874	13	NULL	NULL	0	NULL	malfunction 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiolabelled piperidine derivatives such as ( ( 11 ) C ) MDL 100907 and ( ( 18 ) F ) altanserin have played an important role in diagnosing malfunction in the serotonergic neurotransmission .
	manualset3
128438	6	405874	13	NULL	NULL	0	NULL	serotonergic neurotransmission	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiolabelled piperidine derivatives such as ( ( 11 ) C ) MDL 100907 and ( ( 18 ) F ) altanserin have played an important role in diagnosing malfunction in the serotonergic neurotransmission .
	manualset3
128439	1	405875	13	NULL	NULL	0	NULL	merR homolog	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A merR homolog at 74 minutes on the Escherichia coli genome .
	manualset3
128440	2	405875	13	NULL	NULL	0	NULL	74 minutes	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A merR homolog at 74 minutes on the Escherichia coli genome .
	manualset3
128441	3	405875	13	NULL	NULL	0	NULL	 Escherichia coli genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A merR homolog at 74 minutes on the Escherichia coli genome .
	manualset3
128442	1	405876	13	NULL	NULL	0	NULL	Radioligand binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioligand binding to serotonin-1A and serotonin-1B sites with ( 3H ) 8-OH-DPAT and 125I-cyanopindolol , respectively , after lesions of serotonin axons or depletion of serotonin was not increased , despite a marked increase in ( 3H ) dihydroalprenolol binding in the same tissues .
	manualset3
128443	2	405876	13	NULL	NULL	0	NULL	serotonin-1A sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioligand binding to serotonin-1A and serotonin-1B sites with ( 3H ) 8-OH-DPAT and 125I-cyanopindolol , respectively , after lesions of serotonin axons or depletion of serotonin was not increased , despite a marked increase in ( 3H ) dihydroalprenolol binding in the same tissues .
	manualset3
128444	3	405876	13	NULL	NULL	0	NULL	serotonin-1B sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioligand binding to serotonin-1A and serotonin-1B sites with ( 3H ) 8-OH-DPAT and 125I-cyanopindolol , respectively , after lesions of serotonin axons or depletion of serotonin was not increased , despite a marked increase in ( 3H ) dihydroalprenolol binding in the same tissues .
	manualset3
128445	4	405876	13	NULL	NULL	0	NULL	( 3H ) 8-OH-DPAT	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioligand binding to serotonin-1A and serotonin-1B sites with ( 3H ) 8-OH-DPAT and 125I-cyanopindolol , respectively , after lesions of serotonin axons or depletion of serotonin was not increased , despite a marked increase in ( 3H ) dihydroalprenolol binding in the same tissues .
	manualset3
128446	5	405876	13	NULL	NULL	0	NULL	125I-cyanopindolol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioligand binding to serotonin-1A and serotonin-1B sites with ( 3H ) 8-OH-DPAT and 125I-cyanopindolol , respectively , after lesions of serotonin axons or depletion of serotonin was not increased , despite a marked increase in ( 3H ) dihydroalprenolol binding in the same tissues .
	manualset3
128447	6	405876	13	NULL	NULL	0	NULL	lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioligand binding to serotonin-1A and serotonin-1B sites with ( 3H ) 8-OH-DPAT and 125I-cyanopindolol , respectively , after lesions of serotonin axons or depletion of serotonin was not increased , despite a marked increase in ( 3H ) dihydroalprenolol binding in the same tissues .
	manualset3
128448	7	405876	13	NULL	NULL	0	NULL	serotonin axons 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioligand binding to serotonin-1A and serotonin-1B sites with ( 3H ) 8-OH-DPAT and 125I-cyanopindolol , respectively , after lesions of serotonin axons or depletion of serotonin was not increased , despite a marked increase in ( 3H ) dihydroalprenolol binding in the same tissues .
	manualset3
128449	8	405876	13	NULL	NULL	0	NULL	depletion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioligand binding to serotonin-1A and serotonin-1B sites with ( 3H ) 8-OH-DPAT and 125I-cyanopindolol , respectively , after lesions of serotonin axons or depletion of serotonin was not increased , despite a marked increase in ( 3H ) dihydroalprenolol binding in the same tissues .
	manualset3
128450	9	405876	13	NULL	NULL	0	NULL	serotonin 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioligand binding to serotonin-1A and serotonin-1B sites with ( 3H ) 8-OH-DPAT and 125I-cyanopindolol , respectively , after lesions of serotonin axons or depletion of serotonin was not increased , despite a marked increase in ( 3H ) dihydroalprenolol binding in the same tissues .
	manualset3
128451	10	405876	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioligand binding to serotonin-1A and serotonin-1B sites with ( 3H ) 8-OH-DPAT and 125I-cyanopindolol , respectively , after lesions of serotonin axons or depletion of serotonin was not increased , despite a marked increase in ( 3H ) dihydroalprenolol binding in the same tissues .
	manualset3
128452	11	405876	13	NULL	NULL	0	NULL	( 3H ) dihydroalprenolol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioligand binding to serotonin-1A and serotonin-1B sites with ( 3H ) 8-OH-DPAT and 125I-cyanopindolol , respectively , after lesions of serotonin axons or depletion of serotonin was not increased , despite a marked increase in ( 3H ) dihydroalprenolol binding in the same tissues .
	manualset3
128453	12	405876	13	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioligand binding to serotonin-1A and serotonin-1B sites with ( 3H ) 8-OH-DPAT and 125I-cyanopindolol , respectively , after lesions of serotonin axons or depletion of serotonin was not increased , despite a marked increase in ( 3H ) dihydroalprenolol binding in the same tissues .
	manualset3
128454	13	405876	13	NULL	NULL	0	NULL	tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioligand binding to serotonin-1A and serotonin-1B sites with ( 3H ) 8-OH-DPAT and 125I-cyanopindolol , respectively , after lesions of serotonin axons or depletion of serotonin was not increased , despite a marked increase in ( 3H ) dihydroalprenolol binding in the same tissues .
	manualset3
128455	1	405877	13	NULL	NULL	0	NULL	Radiosensitisation studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiosensitisation studies with SR-2508 ( i.v. ) have been performed in a similar way for comparison purposes .
	manualset3
128456	2	405877	13	NULL	NULL	0	NULL	SR-2508	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiosensitisation studies with SR-2508 ( i.v. ) have been performed in a similar way for comparison purposes .
	manualset3
128457	3	405877	13	NULL	NULL	0	NULL	similar way	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiosensitisation studies with SR-2508 ( i.v. ) have been performed in a similar way for comparison purposes .
	manualset3
128458	4	405877	13	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiosensitisation studies with SR-2508 ( i.v. ) have been performed in a similar way for comparison purposes .
	manualset3
128459	5	405877	13	NULL	NULL	0	NULL	purposes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiosensitisation studies with SR-2508 ( i.v. ) have been performed in a similar way for comparison purposes .
	manualset3
128460	1	405878	13	NULL	NULL	0	NULL	Radiosensitization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiosensitization by nicotinamide in tumors and normal tissues : the importance of tissue oxygenation status .
	manualset3
128461	2	405878	13	NULL	NULL	0	NULL	nicotinamide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiosensitization by nicotinamide in tumors and normal tissues : the importance of tissue oxygenation status .
	manualset3
128462	3	405878	13	NULL	NULL	0	NULL	tumors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiosensitization by nicotinamide in tumors and normal tissues : the importance of tissue oxygenation status .
	manualset3
128463	4	405878	13	NULL	NULL	0	NULL	tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiosensitization by nicotinamide in tumors and normal tissues : the importance of tissue oxygenation status .
	manualset3
128464	5	405878	13	NULL	NULL	0	NULL	importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiosensitization by nicotinamide in tumors and normal tissues : the importance of tissue oxygenation status .
	manualset3
128465	6	405878	13	NULL	NULL	0	NULL	tissue oxygenation status 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiosensitization by nicotinamide in tumors and normal tissues : the importance of tissue oxygenation status .
	manualset3
128466	1	405879	13	NULL	NULL	0	NULL	Radiosynthesis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiosynthesis and in vivo evaluation of ( 11C ) MP-10 as a PET probe for imaging PDE10A in rodent and non-human primate brain .
	manualset3
128467	2	405879	13	NULL	NULL	0	NULL	evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiosynthesis and in vivo evaluation of ( 11C ) MP-10 as a PET probe for imaging PDE10A in rodent and non-human primate brain .
	manualset3
128468	3	405879	13	NULL	NULL	0	NULL	( 11C ) MP-10	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiosynthesis and in vivo evaluation of ( 11C ) MP-10 as a PET probe for imaging PDE10A in rodent and non-human primate brain .
	manualset3
128469	4	405879	13	NULL	NULL	0	NULL	PET probe 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiosynthesis and in vivo evaluation of ( 11C ) MP-10 as a PET probe for imaging PDE10A in rodent and non-human primate brain .
	manualset3
128470	5	405879	13	NULL	NULL	0	NULL	imaging 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiosynthesis and in vivo evaluation of ( 11C ) MP-10 as a PET probe for imaging PDE10A in rodent and non-human primate brain .
	manualset3
128471	6	405879	13	NULL	NULL	0	NULL	PDE10A 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiosynthesis and in vivo evaluation of ( 11C ) MP-10 as a PET probe for imaging PDE10A in rodent and non-human primate brain .
	manualset3
128472	7	405879	13	NULL	NULL	0	NULL	rodent brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiosynthesis and in vivo evaluation of ( 11C ) MP-10 as a PET probe for imaging PDE10A in rodent and non-human primate brain .
	manualset3
128473	8	405879	13	NULL	NULL	0	NULL	non-human primate brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiosynthesis and in vivo evaluation of ( 11C ) MP-10 as a PET probe for imaging PDE10A in rodent and non-human primate brain .
	manualset3
128474	1	405880	13	NULL	NULL	0	NULL	Rainfall 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Rainfall and tillage effects on transport of fecal bacteria and sex hormones 17beta-estradiol and testosterone from broiler litter applications to a Georgia Piedmont Ultisol .
	manualset3
128475	2	405880	13	NULL	NULL	0	NULL	tillage 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rainfall and tillage effects on transport of fecal bacteria and sex hormones 17beta-estradiol and testosterone from broiler litter applications to a Georgia Piedmont Ultisol .
	manualset3
128476	3	405880	13	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rainfall and tillage effects on transport of fecal bacteria and sex hormones 17beta-estradiol and testosterone from broiler litter applications to a Georgia Piedmont Ultisol .
	manualset3
128477	4	405880	13	NULL	NULL	0	NULL	transport	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rainfall and tillage effects on transport of fecal bacteria and sex hormones 17beta-estradiol and testosterone from broiler litter applications to a Georgia Piedmont Ultisol .
	manualset3
128478	5	405880	13	NULL	NULL	0	NULL	fecal bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rainfall and tillage effects on transport of fecal bacteria and sex hormones 17beta-estradiol and testosterone from broiler litter applications to a Georgia Piedmont Ultisol .
	manualset3
128479	6	405880	13	NULL	NULL	0	NULL	sex hormones	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rainfall and tillage effects on transport of fecal bacteria and sex hormones 17beta-estradiol and testosterone from broiler litter applications to a Georgia Piedmont Ultisol .
	manualset3
128480	7	405880	13	NULL	NULL	0	NULL	17beta-estradiol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rainfall and tillage effects on transport of fecal bacteria and sex hormones 17beta-estradiol and testosterone from broiler litter applications to a Georgia Piedmont Ultisol .
	manualset3
128481	8	405880	13	NULL	NULL	0	NULL	testosterone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rainfall and tillage effects on transport of fecal bacteria and sex hormones 17beta-estradiol and testosterone from broiler litter applications to a Georgia Piedmont Ultisol .
	manualset3
128482	9	405880	13	NULL	NULL	0	NULL	 broiler litter applications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rainfall and tillage effects on transport of fecal bacteria and sex hormones 17beta-estradiol and testosterone from broiler litter applications to a Georgia Piedmont Ultisol .
	manualset3
128483	10	405880	13	NULL	NULL	0	NULL	Georgia Piedmont Ultisol	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Rainfall and tillage effects on transport of fecal bacteria and sex hormones 17beta-estradiol and testosterone from broiler litter applications to a Georgia Piedmont Ultisol .
	manualset3
128484	1	405881	13	NULL	NULL	0	NULL	Ralstonia eutropha JMP134 ( pJP4 )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ralstonia eutropha JMP134 ( pJP4 ) harbors two functional gene clusters for the degradation of chlorocatechols , i.e. tfdCDEF ( in short : tfd ( I ) ) and tfdD ( II ) C ( II ) E ( II ) F ( II ) ( in short : tfd ( II ) ) , which are both present on the catabolic plasmid pJP4 .
	manualset3
128486	3	405881	13	NULL	NULL	0	NULL	two functional gene clusters	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ralstonia eutropha JMP134 ( pJP4 ) harbors two functional gene clusters for the degradation of chlorocatechols , i.e. tfdCDEF ( in short : tfd ( I ) ) and tfdD ( II ) C ( II ) E ( II ) F ( II ) ( in short : tfd ( II ) ) , which are both present on the catabolic plasmid pJP4 .
	manualset3
128487	4	405881	13	NULL	NULL	0	NULL	degradation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ralstonia eutropha JMP134 ( pJP4 ) harbors two functional gene clusters for the degradation of chlorocatechols , i.e. tfdCDEF ( in short : tfd ( I ) ) and tfdD ( II ) C ( II ) E ( II ) F ( II ) ( in short : tfd ( II ) ) , which are both present on the catabolic plasmid pJP4 .
	manualset3
128488	5	405881	13	NULL	NULL	0	NULL	chlorocatechols	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ralstonia eutropha JMP134 ( pJP4 ) harbors two functional gene clusters for the degradation of chlorocatechols , i.e. tfdCDEF ( in short : tfd ( I ) ) and tfdD ( II ) C ( II ) E ( II ) F ( II ) ( in short : tfd ( II ) ) , which are both present on the catabolic plasmid pJP4 .
	manualset3
128489	6	405881	13	NULL	NULL	0	NULL	tfdCDEF ( in short : tfd ( I ) )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Ralstonia eutropha JMP134 ( pJP4 ) harbors two functional gene clusters for the degradation of chlorocatechols , i.e. tfdCDEF ( in short : tfd ( I ) ) and tfdD ( II ) C ( II ) E ( II ) F ( II ) ( in short : tfd ( II ) ) , which are both present on the catabolic plasmid pJP4 .
	manualset3
128490	7	405881	13	NULL	NULL	0	NULL	tfdD ( II ) C ( II ) E ( II ) F ( II ) ( in short : tfd ( II ) ) 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Ralstonia eutropha JMP134 ( pJP4 ) harbors two functional gene clusters for the degradation of chlorocatechols , i.e. tfdCDEF ( in short : tfd ( I ) ) and tfdD ( II ) C ( II ) E ( II ) F ( II ) ( in short : tfd ( II ) ) , which are both present on the catabolic plasmid pJP4 .
	manualset3
128491	8	405881	13	NULL	NULL	0	NULL	catabolic plasmid pJP4	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Ralstonia eutropha JMP134 ( pJP4 ) harbors two functional gene clusters for the degradation of chlorocatechols , i.e. tfdCDEF ( in short : tfd ( I ) ) and tfdD ( II ) C ( II ) E ( II ) F ( II ) ( in short : tfd ( II ) ) , which are both present on the catabolic plasmid pJP4 .
	manualset3
128492	1	405882	13	NULL	NULL	0	NULL	Raman spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Raman spectroscopy is a nondestructive optical technique that enables real-time tissue identification and classification and has proved to be a powerful diagnostic tool in a large number of studies .
	manualset3
128493	2	405882	13	NULL	NULL	0	NULL	nondestructive optical technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Raman spectroscopy is a nondestructive optical technique that enables real-time tissue identification and classification and has proved to be a powerful diagnostic tool in a large number of studies .
	manualset3
128494	3	405882	13	NULL	NULL	0	NULL	real-time tissue identification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Raman spectroscopy is a nondestructive optical technique that enables real-time tissue identification and classification and has proved to be a powerful diagnostic tool in a large number of studies .
	manualset3
128495	4	405882	13	NULL	NULL	0	NULL	classification 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Raman spectroscopy is a nondestructive optical technique that enables real-time tissue identification and classification and has proved to be a powerful diagnostic tool in a large number of studies .
	manualset3
128496	5	405882	13	NULL	NULL	0	NULL	diagnostic tool 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Raman spectroscopy is a nondestructive optical technique that enables real-time tissue identification and classification and has proved to be a powerful diagnostic tool in a large number of studies .
	manualset3
128497	6	405882	13	NULL	NULL	0	NULL	number 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Raman spectroscopy is a nondestructive optical technique that enables real-time tissue identification and classification and has proved to be a powerful diagnostic tool in a large number of studies .
	manualset3
128498	7	405882	13	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Raman spectroscopy is a nondestructive optical technique that enables real-time tissue identification and classification and has proved to be a powerful diagnostic tool in a large number of studies .
	manualset3
128499	1	405883	13	NULL	NULL	0	NULL	method	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for identifying causative chemicals of allergic contact dermatitis using a combination of chemical analysis and patch testing in patients and animal groups : application to a case of rubber boot dermatitis .
	manualset3
128500	2	405883	13	NULL	NULL	0	NULL	causative chemicals 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for identifying causative chemicals of allergic contact dermatitis using a combination of chemical analysis and patch testing in patients and animal groups : application to a case of rubber boot dermatitis .
	manualset3
128501	3	405883	13	NULL	NULL	0	NULL	allergic contact dermatitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for identifying causative chemicals of allergic contact dermatitis using a combination of chemical analysis and patch testing in patients and animal groups : application to a case of rubber boot dermatitis .
	manualset3
128502	4	405883	13	NULL	NULL	0	NULL	 combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for identifying causative chemicals of allergic contact dermatitis using a combination of chemical analysis and patch testing in patients and animal groups : application to a case of rubber boot dermatitis .
	manualset3
128503	5	405883	13	NULL	NULL	0	NULL	chemical analysis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for identifying causative chemicals of allergic contact dermatitis using a combination of chemical analysis and patch testing in patients and animal groups : application to a case of rubber boot dermatitis .
	manualset3
128504	6	405883	13	NULL	NULL	0	NULL	patch testing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for identifying causative chemicals of allergic contact dermatitis using a combination of chemical analysis and patch testing in patients and animal groups : application to a case of rubber boot dermatitis .
	manualset3
128505	7	405883	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for identifying causative chemicals of allergic contact dermatitis using a combination of chemical analysis and patch testing in patients and animal groups : application to a case of rubber boot dermatitis .
	manualset3
128506	8	405883	13	NULL	NULL	0	NULL	animal groups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for identifying causative chemicals of allergic contact dermatitis using a combination of chemical analysis and patch testing in patients and animal groups : application to a case of rubber boot dermatitis .
	manualset3
128507	9	405883	13	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for identifying causative chemicals of allergic contact dermatitis using a combination of chemical analysis and patch testing in patients and animal groups : application to a case of rubber boot dermatitis .
	manualset3
128508	10	405883	13	NULL	NULL	NULL	NULL	case of rubber boot dermatitis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A method for identifying causative chemicals of allergic contact dermatitis using a combination of chemical analysis and patch testing in patients and animal groups : application to a case of rubber boot dermatitis .
	manualset3
128509	1	405884	13	NULL	NULL	0	NULL	Raman spectroscopic measurements	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Raman and X-ray photoelectron spectroscopic measurements indicate the charge transfer from graphene to PDDA .
	manualset3
128510	2	405884	13	NULL	NULL	0	NULL	X-ray photoelectron spectroscopic measurements	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Raman and X-ray photoelectron spectroscopic measurements indicate the charge transfer from graphene to PDDA .
	manualset3
128511	3	405884	13	NULL	NULL	0	NULL	charge transfer	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Raman and X-ray photoelectron spectroscopic measurements indicate the charge transfer from graphene to PDDA .
	manualset3
128512	4	405884	13	NULL	NULL	0	NULL	graphene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Raman and X-ray photoelectron spectroscopic measurements indicate the charge transfer from graphene to PDDA .
	manualset3
128513	5	405884	13	NULL	NULL	0	NULL	PDDA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Raman and X-ray photoelectron spectroscopic measurements indicate the charge transfer from graphene to PDDA .
	manualset3
128514	1	405885	13	NULL	NULL	0	NULL	Random mutagenesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Random mutagenesis of residues within a surface-exposed region of the major AAV9 capsid protein yielded a capsid library with mutations clustered at the icosahedral threefold symmetry axis .
	manualset3
128515	2	405885	13	NULL	NULL	0	NULL	residues 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Random mutagenesis of residues within a surface-exposed region of the major AAV9 capsid protein yielded a capsid library with mutations clustered at the icosahedral threefold symmetry axis .
	manualset3
128516	3	405885	13	NULL	NULL	0	NULL	surface-exposed region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Random mutagenesis of residues within a surface-exposed region of the major AAV9 capsid protein yielded a capsid library with mutations clustered at the icosahedral threefold symmetry axis .
	manualset3
128517	4	405885	13	NULL	NULL	0	NULL	AAV9 capsid protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Random mutagenesis of residues within a surface-exposed region of the major AAV9 capsid protein yielded a capsid library with mutations clustered at the icosahedral threefold symmetry axis .
	manualset3
128518	5	405885	13	NULL	NULL	0	NULL	capsid library	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Random mutagenesis of residues within a surface-exposed region of the major AAV9 capsid protein yielded a capsid library with mutations clustered at the icosahedral threefold symmetry axis .
	manualset3
128519	6	405885	13	NULL	NULL	0	NULL	mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Random mutagenesis of residues within a surface-exposed region of the major AAV9 capsid protein yielded a capsid library with mutations clustered at the icosahedral threefold symmetry axis .
	manualset3
128520	7	405885	13	NULL	NULL	0	NULL	icosahedral threefold symmetry axis	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Random mutagenesis of residues within a surface-exposed region of the major AAV9 capsid protein yielded a capsid library with mutations clustered at the icosahedral threefold symmetry axis .
	manualset3
128521	1	405886	13	NULL	NULL	0	NULL	trial	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Randomised trial comparing biweekly oxaliplatin plus oral capecitabine versus oxaliplatin plus i.v. bolus fluorouracil/leucovorin in metastatic colorectal cancer patients : results of the Southern Italy Cooperative Oncology study 0401 .
	manualset3
128522	2	405886	13	NULL	NULL	0	NULL	oxaliplatin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Randomised trial comparing biweekly oxaliplatin plus oral capecitabine versus oxaliplatin plus i.v. bolus fluorouracil/leucovorin in metastatic colorectal cancer patients : results of the Southern Italy Cooperative Oncology study 0401 .
	manualset3
128523	3	405886	13	NULL	NULL	0	NULL	oral capecitabine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Randomised trial comparing biweekly oxaliplatin plus oral capecitabine versus oxaliplatin plus i.v. bolus fluorouracil/leucovorin in metastatic colorectal cancer patients : results of the Southern Italy Cooperative Oncology study 0401 .
	manualset3
128524	4	405886	13	NULL	NULL	0	NULL	oxaliplatin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Randomised trial comparing biweekly oxaliplatin plus oral capecitabine versus oxaliplatin plus i.v. bolus fluorouracil/leucovorin in metastatic colorectal cancer patients : results of the Southern Italy Cooperative Oncology study 0401 .
	manualset3
128525	5	405886	13	NULL	NULL	0	NULL	fluorouracil	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Randomised trial comparing biweekly oxaliplatin plus oral capecitabine versus oxaliplatin plus i.v. bolus fluorouracil/leucovorin in metastatic colorectal cancer patients : results of the Southern Italy Cooperative Oncology study 0401 .
	manualset3
128526	6	405886	13	NULL	NULL	0	NULL	leucovorin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Randomised trial comparing biweekly oxaliplatin plus oral capecitabine versus oxaliplatin plus i.v. bolus fluorouracil/leucovorin in metastatic colorectal cancer patients : results of the Southern Italy Cooperative Oncology study 0401 .
	manualset3
128527	7	405886	13	NULL	NULL	0	NULL	metastatic colorectal cancer patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Randomised trial comparing biweekly oxaliplatin plus oral capecitabine versus oxaliplatin plus i.v. bolus fluorouracil/leucovorin in metastatic colorectal cancer patients : results of the Southern Italy Cooperative Oncology study 0401 .
	manualset3
128528	8	405886	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Randomised trial comparing biweekly oxaliplatin plus oral capecitabine versus oxaliplatin plus i.v. bolus fluorouracil/leucovorin in metastatic colorectal cancer patients : results of the Southern Italy Cooperative Oncology study 0401 .
	manualset3
128529	9	405886	13	NULL	NULL	0	NULL	Southern Italy Cooperative Oncology study 0401 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Randomised trial comparing biweekly oxaliplatin plus oral capecitabine versus oxaliplatin plus i.v. bolus fluorouracil/leucovorin in metastatic colorectal cancer patients : results of the Southern Italy Cooperative Oncology study 0401 .
	manualset3
128530	1	405887	13	NULL	NULL	0	NULL	Range of motion	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Range of motion and grip power were reduced compared to the unaffected hand , but only loss of supination and ulnar deviation correlated with an unsatisfactory subjective result .
	manualset3
128531	2	405887	13	NULL	NULL	0	NULL	grip power	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Range of motion and grip power were reduced compared to the unaffected hand , but only loss of supination and ulnar deviation correlated with an unsatisfactory subjective result .
	manualset3
128532	3	405887	13	NULL	NULL	0	NULL	hand	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Range of motion and grip power were reduced compared to the unaffected hand , but only loss of supination and ulnar deviation correlated with an unsatisfactory subjective result .
	manualset3
128533	4	405887	13	NULL	NULL	0	NULL	loss of supination 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Range of motion and grip power were reduced compared to the unaffected hand , but only loss of supination and ulnar deviation correlated with an unsatisfactory subjective result .
	manualset3
128534	5	405887	13	NULL	NULL	0	NULL	ulnar deviation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Range of motion and grip power were reduced compared to the unaffected hand , but only loss of supination and ulnar deviation correlated with an unsatisfactory subjective result .
	manualset3
128535	6	405887	13	NULL	NULL	0	NULL	result 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Range of motion and grip power were reduced compared to the unaffected hand , but only loss of supination and ulnar deviation correlated with an unsatisfactory subjective result .
	manualset3
128536	1	405888	13	NULL	NULL	0	NULL	Ranking	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ranking the carcinogenic potential of chemical mixtures : the integral search system and its use in evaluating hazardous waste sites .
	manualset3
128537	2	405888	13	NULL	NULL	NULL	NULL	carcinogenic potential	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ranking the carcinogenic potential of chemical mixtures : the integral search system and its use in evaluating hazardous waste sites .
	manualset3
128538	3	405888	13	NULL	NULL	0	NULL	chemical mixtures	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ranking the carcinogenic potential of chemical mixtures : the integral search system and its use in evaluating hazardous waste sites .
	manualset3
128539	4	405888	13	NULL	NULL	0	NULL	integral search system	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ranking the carcinogenic potential of chemical mixtures : the integral search system and its use in evaluating hazardous waste sites .
	manualset3
128540	5	405888	13	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ranking the carcinogenic potential of chemical mixtures : the integral search system and its use in evaluating hazardous waste sites .
	manualset3
128541	6	405888	13	NULL	NULL	0	NULL	hazardous waste sites 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Ranking the carcinogenic potential of chemical mixtures : the integral search system and its use in evaluating hazardous waste sites .
	manualset3
128542	1	405889	13	NULL	NULL	0	NULL	Rapamycin 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapamycin , besides inducing autophagy , also increased Akt and CREB ( cAMP response element-binding protein ) phosphorylation in the same cells .
	manualset3
128543	2	405889	13	NULL	NULL	0	NULL	autophagy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapamycin , besides inducing autophagy , also increased Akt and CREB ( cAMP response element-binding protein ) phosphorylation in the same cells .
	manualset3
128544	3	405889	13	NULL	NULL	0	NULL	Akt	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapamycin , besides inducing autophagy , also increased Akt and CREB ( cAMP response element-binding protein ) phosphorylation in the same cells .
	manualset3
128545	4	405889	13	NULL	NULL	0	NULL	CREB ( cAMP response element-binding protein ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapamycin , besides inducing autophagy , also increased Akt and CREB ( cAMP response element-binding protein ) phosphorylation in the same cells .
	manualset3
128546	5	405889	13	NULL	NULL	0	NULL	phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapamycin , besides inducing autophagy , also increased Akt and CREB ( cAMP response element-binding protein ) phosphorylation in the same cells .
	manualset3
128547	6	405889	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapamycin , besides inducing autophagy , also increased Akt and CREB ( cAMP response element-binding protein ) phosphorylation in the same cells .
	manualset3
128548	1	405890	13	NULL	NULL	0	NULL	LC-MS method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid and sensitive LC-MS method for pharmacokinetic study of vinorelbine in rats .
	manualset3
128549	2	405890	13	NULL	NULL	0	NULL	pharmacokinetic study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid and sensitive LC-MS method for pharmacokinetic study of vinorelbine in rats .
	manualset3
128550	3	405890	13	NULL	NULL	0	NULL	vinorelbine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid and sensitive LC-MS method for pharmacokinetic study of vinorelbine in rats .
	manualset3
128551	4	405890	13	NULL	NULL	0	NULL	rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid and sensitive LC-MS method for pharmacokinetic study of vinorelbine in rats .
	manualset3
128552	1	405891	13	NULL	NULL	0	NULL	method	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for preparing five - or six-membered heterocyclic compounds from enyne carbonates via palladium catalysis was developed .
	manualset3
128553	2	405891	13	NULL	NULL	0	NULL	five-membered heterocyclic compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for preparing five - or six-membered heterocyclic compounds from enyne carbonates via palladium catalysis was developed .
	manualset3
128554	3	405891	13	NULL	NULL	0	NULL	six-membered heterocyclic compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for preparing five - or six-membered heterocyclic compounds from enyne carbonates via palladium catalysis was developed .
	manualset3
128555	4	405891	13	NULL	NULL	0	NULL	enyne carbonates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for preparing five - or six-membered heterocyclic compounds from enyne carbonates via palladium catalysis was developed .
	manualset3
128556	5	405891	13	NULL	NULL	0	NULL	palladium catalysis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for preparing five - or six-membered heterocyclic compounds from enyne carbonates via palladium catalysis was developed .
	manualset3
128557	1	405892	13	NULL	NULL	0	NULL	Rapid automated detection 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid automated detection of hepatitis B surface antigen with the Centria automated radioimmunoassay system .
	manualset3
128558	2	405892	13	NULL	NULL	0	NULL	hepatitis B surface antigen	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid automated detection of hepatitis B surface antigen with the Centria automated radioimmunoassay system .
	manualset3
128559	3	405892	13	NULL	NULL	0	NULL	Centria automated radioimmunoassay system	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid automated detection of hepatitis B surface antigen with the Centria automated radioimmunoassay system .
	manualset3
128560	1	405893	13	NULL	NULL	0	NULL	Rapid calcium release 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid calcium release and proton uptake at the disk membrane of isolated cattle rod outer segments .
	manualset3
128561	2	405893	13	NULL	NULL	0	NULL	proton uptake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid calcium release and proton uptake at the disk membrane of isolated cattle rod outer segments .
	manualset3
128562	3	405893	13	NULL	NULL	0	NULL	disk membrane 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid calcium release and proton uptake at the disk membrane of isolated cattle rod outer segments .
	manualset3
128563	4	405893	13	NULL	NULL	0	NULL	cattle rod outer segments	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid calcium release and proton uptake at the disk membrane of isolated cattle rod outer segments .
	manualset3
128565	1	405894	13	NULL	NULL	0	NULL	Rapid compliance changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid compliance changes were accompanied by significantly decreased collagen and fibronectin levels and increased gelatinase ( MMP-2 and -9 ) abundance and activation .
	manualset3
128566	2	405894	13	NULL	NULL	0	NULL	collagen levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid compliance changes were accompanied by significantly decreased collagen and fibronectin levels and increased gelatinase ( MMP-2 and -9 ) abundance and activation .
	manualset3
128567	3	405894	13	NULL	NULL	0	NULL	fibronectin levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid compliance changes were accompanied by significantly decreased collagen and fibronectin levels and increased gelatinase ( MMP-2 and -9 ) abundance and activation .
	manualset3
128568	4	405894	13	NULL	NULL	0	NULL	gelatinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid compliance changes were accompanied by significantly decreased collagen and fibronectin levels and increased gelatinase ( MMP-2 and -9 ) abundance and activation .
	manualset3
128569	5	405894	13	NULL	NULL	0	NULL	MMP-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid compliance changes were accompanied by significantly decreased collagen and fibronectin levels and increased gelatinase ( MMP-2 and -9 ) abundance and activation .
	manualset3
128570	6	405894	13	NULL	NULL	NULL	NULL	MMP-9	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Rapid compliance changes were accompanied by significantly decreased collagen and fibronectin levels and increased gelatinase ( MMP-2 and -9 ) abundance and activation .
	manualset3
128571	7	405894	13	NULL	NULL	0	NULL	abundance	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid compliance changes were accompanied by significantly decreased collagen and fibronectin levels and increased gelatinase ( MMP-2 and -9 ) abundance and activation .
	manualset3
128572	8	405894	13	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid compliance changes were accompanied by significantly decreased collagen and fibronectin levels and increased gelatinase ( MMP-2 and -9 ) abundance and activation .
	manualset3
128573	1	405895	13	NULL	NULL	0	NULL	Rapid construction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid construction of empirical RNA fitness landscapes .
	manualset3
128574	2	405895	13	NULL	NULL	0	NULL	RNA fitness landscapes	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid construction of empirical RNA fitness landscapes .
	manualset3
128575	1	405896	13	NULL	NULL	0	NULL	Rapid detection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid detection and prenatal diagnosis of beta-thalassaemia : studies in Indian and Cypriot populations in the UK .
	manualset3
128576	2	405896	13	NULL	NULL	0	NULL	prenatal diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid detection and prenatal diagnosis of beta-thalassaemia : studies in Indian and Cypriot populations in the UK .
	manualset3
128577	3	405896	13	NULL	NULL	0	NULL	beta-thalassaemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid detection and prenatal diagnosis of beta-thalassaemia : studies in Indian and Cypriot populations in the UK .
	manualset3
128578	4	405896	13	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid detection and prenatal diagnosis of beta-thalassaemia : studies in Indian and Cypriot populations in the UK .
	manualset3
128579	5	405896	13	NULL	NULL	0	NULL	Indian populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid detection and prenatal diagnosis of beta-thalassaemia : studies in Indian and Cypriot populations in the UK .
	manualset3
128580	6	405896	13	NULL	NULL	0	NULL	Cypriot populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid detection and prenatal diagnosis of beta-thalassaemia : studies in Indian and Cypriot populations in the UK .
	manualset3
128581	7	405896	13	NULL	NULL	0	NULL	UK	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid detection and prenatal diagnosis of beta-thalassaemia : studies in Indian and Cypriot populations in the UK .
	manualset3
128582	1	405897	13	NULL	NULL	0	NULL	Rapid detection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid detection of a critical change in tissue oxygenation could enable earlier and more successful surgical intervention when such problems arise .
	manualset3
128583	2	405897	13	NULL	NULL	0	NULL	critical change 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid detection of a critical change in tissue oxygenation could enable earlier and more successful surgical intervention when such problems arise .
	manualset3
128584	3	405897	13	NULL	NULL	0	NULL	tissue oxygenation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid detection of a critical change in tissue oxygenation could enable earlier and more successful surgical intervention when such problems arise .
	manualset3
128585	4	405897	13	NULL	NULL	0	NULL	surgical intervention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid detection of a critical change in tissue oxygenation could enable earlier and more successful surgical intervention when such problems arise .
	manualset3
128586	5	405897	13	NULL	NULL	0	NULL	 problems 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid detection of a critical change in tissue oxygenation could enable earlier and more successful surgical intervention when such problems arise .
	manualset3
128587	1	405898	13	NULL	NULL	0	NULL	Rapid detection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid detection of oseltamivir resistance in severe infection is essential for patients to receive maximum therapeutic benefit .
	manualset3
128588	2	405898	13	NULL	NULL	0	NULL	oseltamivir resistance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid detection of oseltamivir resistance in severe infection is essential for patients to receive maximum therapeutic benefit .
	manualset3
128589	3	405898	13	NULL	NULL	0	NULL	severe infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid detection of oseltamivir resistance in severe infection is essential for patients to receive maximum therapeutic benefit .
	manualset3
128590	4	405898	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid detection of oseltamivir resistance in severe infection is essential for patients to receive maximum therapeutic benefit .
	manualset3
128591	5	405898	13	NULL	NULL	0	NULL	therapeutic benefit 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid detection of oseltamivir resistance in severe infection is essential for patients to receive maximum therapeutic benefit .
	manualset3
128592	1	405899	13	NULL	NULL	0	NULL	Rapid eye movement ( REM ) sleep	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid eye movement ( REM ) sleep is a behavioral state characterized by cerebral cortical activation with dreaming as an associated behavior .
	manualset3
128593	2	405899	13	NULL	NULL	0	NULL	behavioral state	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid eye movement ( REM ) sleep is a behavioral state characterized by cerebral cortical activation with dreaming as an associated behavior .
	manualset3
128594	3	405899	13	NULL	NULL	0	NULL	cerebral cortical activation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid eye movement ( REM ) sleep is a behavioral state characterized by cerebral cortical activation with dreaming as an associated behavior .
	manualset3
128595	4	405899	13	NULL	NULL	0	NULL	behavior	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid eye movement ( REM ) sleep is a behavioral state characterized by cerebral cortical activation with dreaming as an associated behavior .
	manualset3
128596	1	405900	13	NULL	NULL	0	NULL	Rapid immunochromatographic test 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid immunochromatographic test using recombinant SAG2 for detection of antibodies against Toxoplasma gondii in cats .
	manualset3
128597	2	405900	13	NULL	NULL	0	NULL	recombinant SAG2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid immunochromatographic test using recombinant SAG2 for detection of antibodies against Toxoplasma gondii in cats .
	manualset3
128598	3	405900	13	NULL	NULL	0	NULL	detection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid immunochromatographic test using recombinant SAG2 for detection of antibodies against Toxoplasma gondii in cats .
	manualset3
128599	4	405900	13	NULL	NULL	0	NULL	antibodies 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid immunochromatographic test using recombinant SAG2 for detection of antibodies against Toxoplasma gondii in cats .
	manualset3
128600	5	405900	13	NULL	NULL	0	NULL	Toxoplasma gondii	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid immunochromatographic test using recombinant SAG2 for detection of antibodies against Toxoplasma gondii in cats .
	manualset3
128601	6	405900	13	NULL	NULL	0	NULL	cats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid immunochromatographic test using recombinant SAG2 for detection of antibodies against Toxoplasma gondii in cats .
	manualset3
128602	1	405901	13	NULL	NULL	0	NULL	method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128603	2	405901	13	NULL	NULL	0	NULL	simultaneous screening	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128604	3	405901	13	NULL	NULL	0	NULL	quantification 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128605	4	405901	13	NULL	NULL	0	NULL	fentanyls alfentanil	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128606	5	405901	13	NULL	NULL	0	NULL	fentanyl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128607	6	405901	13	NULL	NULL	0	NULL	p-fluorofentanyl 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128608	7	405901	13	NULL	NULL	0	NULL	cis-3-methylfentanyl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128609	8	405901	13	NULL	NULL	0	NULL	trans-3-methylfentanyl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128610	9	405901	13	NULL	NULL	0	NULL	alpha-methylfentanyl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128611	10	405901	13	NULL	NULL	0	NULL	norfentanyl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128612	11	405901	13	NULL	NULL	0	NULL	remifentanil	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128613	12	405901	13	NULL	NULL	0	NULL	sufentanil	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128614	13	405901	13	NULL	NULL	0	NULL	opioid drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128615	14	405901	13	NULL	NULL	0	NULL	6-acetylmorphine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128616	15	405901	13	NULL	NULL	0	NULL	buprenorphine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128617	16	405901	13	NULL	NULL	0	NULL	codeine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128618	17	405901	13	NULL	NULL	0	NULL	dextropropoxyphene	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128619	18	405901	13	NULL	NULL	0	NULL	ethylmorphine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128620	19	405901	13	NULL	NULL	0	NULL	heroin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128621	20	405901	13	NULL	NULL	0	NULL	methadone 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128622	21	405901	13	NULL	NULL	0	NULL	morphine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128623	22	405901	13	NULL	NULL	0	NULL	naloxone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128624	23	405901	13	NULL	NULL	0	NULL	naltrexone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128625	24	405901	13	NULL	NULL	0	NULL	norbuprenorphine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128626	25	405901	13	NULL	NULL	0	NULL	normethadone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128627	26	405901	13	NULL	NULL	0	NULL	oxycodone 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128628	27	405901	13	NULL	NULL	0	NULL	pentazocine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128629	28	405901	13	NULL	NULL	0	NULL	pethidine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128630	29	405901	13	NULL	NULL	0	NULL	tramadol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128631	30	405901	13	NULL	NULL	0	NULL	post-mortem blood 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128632	31	405901	13	NULL	NULL	0	NULL	urine samples	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128633	32	405901	13	NULL	NULL	0	NULL	LC-MS/MS	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for simultaneous screening and quantification was developed for the fentanyls alfentanil , fentanyl , p-fluorofentanyl , cis-3-methylfentanyl , trans-3-methylfentanyl , alpha-methylfentanyl , norfentanyl , remifentanil , sufentanil , and the other opioid drugs 6-acetylmorphine , buprenorphine , codeine , dextropropoxyphene , ethylmorphine , heroin , methadone , morphine , naloxone , naltrexone , norbuprenorphine , normethadone , oxycodone , pentazocine , pethidine , and tramadol in post-mortem blood and urine samples by LC-MS/MS .
	manualset3
128634	1	405902	13	NULL	NULL	0	NULL	Rapid loss	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid loss of plasma protein in acute surgical conditions .
	manualset3
128635	2	405902	13	NULL	NULL	0	NULL	plasma protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid loss of plasma protein in acute surgical conditions .
	manualset3
128636	3	405902	13	NULL	NULL	0	NULL	acute surgical conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid loss of plasma protein in acute surgical conditions .
	manualset3
128637	1	405903	13	NULL	NULL	0	NULL	Rapid method	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid method for processing soil samples for polymerase chain reaction amplification of specific gene sequences .
	manualset3
128638	2	405903	13	NULL	NULL	0	NULL	processing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid method for processing soil samples for polymerase chain reaction amplification of specific gene sequences .
	manualset3
128639	3	405903	13	NULL	NULL	0	NULL	soil samples 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid method for processing soil samples for polymerase chain reaction amplification of specific gene sequences .
	manualset3
128640	4	405903	13	NULL	NULL	0	NULL	polymerase chain reaction amplification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid method for processing soil samples for polymerase chain reaction amplification of specific gene sequences .
	manualset3
128641	5	405903	13	NULL	NULL	0	NULL	gene sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid method for processing soil samples for polymerase chain reaction amplification of specific gene sequences .
	manualset3
128642	1	405904	13	NULL	NULL	0	NULL	Rapid purification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid purification of recombinant dengue and West Nile virus envelope Domain III proteins by metal affinity membrane chromatography .
	manualset3
128643	2	405904	13	NULL	NULL	0	NULL	recombinant dengue proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid purification of recombinant dengue and West Nile virus envelope Domain III proteins by metal affinity membrane chromatography .
	manualset3
128644	3	405904	13	NULL	NULL	0	NULL	West Nile virus envelope Domain III proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid purification of recombinant dengue and West Nile virus envelope Domain III proteins by metal affinity membrane chromatography .
	manualset3
128645	4	405904	13	NULL	NULL	0	NULL	metal affinity membrane chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid purification of recombinant dengue and West Nile virus envelope Domain III proteins by metal affinity membrane chromatography .
	manualset3
128646	1	405905	13	NULL	NULL	NULL	NULL	Rapid sequence intubation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Rapid sequence intubation is the process involving administration of a sedative ( eg , induction agent ) followed almost immediately by a neuromuscular blocking agent to facilitate endotracheal intubation The purpose of emergency RSI is to make emergent intubation easier and safer , thereby increasing the success rate of intubation while decreasing the complications .
	manualset3
128647	2	405905	13	NULL	NULL	0	NULL	process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid sequence intubation is the process involving administration of a sedative ( eg , induction agent ) followed almost immediately by a neuromuscular blocking agent to facilitate endotracheal intubation The purpose of emergency RSI is to make emergent intubation easier and safer , thereby increasing the success rate of intubation while decreasing the complications .
	manualset3
128648	3	405905	13	NULL	NULL	0	NULL	administration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid sequence intubation is the process involving administration of a sedative ( eg , induction agent ) followed almost immediately by a neuromuscular blocking agent to facilitate endotracheal intubation The purpose of emergency RSI is to make emergent intubation easier and safer , thereby increasing the success rate of intubation while decreasing the complications .
	manualset3
128649	4	405905	13	NULL	NULL	0	NULL	sedative	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid sequence intubation is the process involving administration of a sedative ( eg , induction agent ) followed almost immediately by a neuromuscular blocking agent to facilitate endotracheal intubation The purpose of emergency RSI is to make emergent intubation easier and safer , thereby increasing the success rate of intubation while decreasing the complications .
	manualset3
128650	5	405905	13	NULL	NULL	0	NULL	induction agent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid sequence intubation is the process involving administration of a sedative ( eg , induction agent ) followed almost immediately by a neuromuscular blocking agent to facilitate endotracheal intubation The purpose of emergency RSI is to make emergent intubation easier and safer , thereby increasing the success rate of intubation while decreasing the complications .
	manualset3
128651	6	405905	13	NULL	NULL	0	NULL	neuromuscular blocking agent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid sequence intubation is the process involving administration of a sedative ( eg , induction agent ) followed almost immediately by a neuromuscular blocking agent to facilitate endotracheal intubation The purpose of emergency RSI is to make emergent intubation easier and safer , thereby increasing the success rate of intubation while decreasing the complications .
	manualset3
128652	7	405905	13	NULL	NULL	NULL	NULL	endotracheal intubation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Rapid sequence intubation is the process involving administration of a sedative ( eg , induction agent ) followed almost immediately by a neuromuscular blocking agent to facilitate endotracheal intubation The purpose of emergency RSI is to make emergent intubation easier and safer , thereby increasing the success rate of intubation while decreasing the complications .
	manualset3
128653	8	405905	13	NULL	NULL	0	NULL	purpose 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid sequence intubation is the process involving administration of a sedative ( eg , induction agent ) followed almost immediately by a neuromuscular blocking agent to facilitate endotracheal intubation The purpose of emergency RSI is to make emergent intubation easier and safer , thereby increasing the success rate of intubation while decreasing the complications .
	manualset3
128654	9	405905	13	NULL	NULL	0	NULL	emergency RSI	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid sequence intubation is the process involving administration of a sedative ( eg , induction agent ) followed almost immediately by a neuromuscular blocking agent to facilitate endotracheal intubation The purpose of emergency RSI is to make emergent intubation easier and safer , thereby increasing the success rate of intubation while decreasing the complications .
	manualset3
128655	10	405905	13	NULL	NULL	0	NULL	emergent intubation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid sequence intubation is the process involving administration of a sedative ( eg , induction agent ) followed almost immediately by a neuromuscular blocking agent to facilitate endotracheal intubation The purpose of emergency RSI is to make emergent intubation easier and safer , thereby increasing the success rate of intubation while decreasing the complications .
	manualset3
128656	11	405905	13	NULL	NULL	0	NULL	success rate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid sequence intubation is the process involving administration of a sedative ( eg , induction agent ) followed almost immediately by a neuromuscular blocking agent to facilitate endotracheal intubation The purpose of emergency RSI is to make emergent intubation easier and safer , thereby increasing the success rate of intubation while decreasing the complications .
	manualset3
128657	12	405905	13	NULL	NULL	0	NULL	intubation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid sequence intubation is the process involving administration of a sedative ( eg , induction agent ) followed almost immediately by a neuromuscular blocking agent to facilitate endotracheal intubation The purpose of emergency RSI is to make emergent intubation easier and safer , thereby increasing the success rate of intubation while decreasing the complications .
	manualset3
128658	13	405905	13	NULL	NULL	0	NULL	complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapid sequence intubation is the process involving administration of a sedative ( eg , induction agent ) followed almost immediately by a neuromuscular blocking agent to facilitate endotracheal intubation The purpose of emergency RSI is to make emergent intubation easier and safer , thereby increasing the success rate of intubation while decreasing the complications .
	manualset3
128659	1	405906	13	NULL	NULL	0	NULL	Rare clinical presentation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rare clinical presentation of testicular tumor .
	manualset3
128660	2	405906	13	NULL	NULL	0	NULL	testicular tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rare clinical presentation of testicular tumor .
	manualset3
128661	1	405907	13	NULL	NULL	0	NULL	Rare deviations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rare deviations in serial visual stimulation are accompanied by an occipital N2 in the event-related potential ( the visual mismatch negativity ( vMMN ) ) .
	manualset3
128662	2	405907	13	NULL	NULL	0	NULL	serial visual stimulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rare deviations in serial visual stimulation are accompanied by an occipital N2 in the event-related potential ( the visual mismatch negativity ( vMMN ) ) .
	manualset3
128663	3	405907	13	NULL	NULL	0	NULL	occipital N2	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Rare deviations in serial visual stimulation are accompanied by an occipital N2 in the event-related potential ( the visual mismatch negativity ( vMMN ) ) .
	manualset3
128664	4	405907	13	NULL	NULL	0	NULL	visual mismatch negativity ( vMMN )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rare deviations in serial visual stimulation are accompanied by an occipital N2 in the event-related potential ( the visual mismatch negativity ( vMMN ) ) .
	manualset3
131916	5	405907	13	NULL	NULL	0	NULL	event-related potential 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rare deviations in serial visual stimulation are accompanied by an occipital N2 in the event-related potential ( the visual mismatch negativity ( vMMN ) ) .
	manualset3
128665	1	405908	13	NULL	NULL	0	NULL	AS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Rarely AS is seen in combination with diffuse leiomyomatosis ( DL ) .
	manualset3
128666	2	405908	13	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rarely AS is seen in combination with diffuse leiomyomatosis ( DL ) .
	manualset3
128667	3	405908	13	NULL	NULL	0	NULL	diffuse leiomyomatosis ( DL )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Rarely AS is seen in combination with diffuse leiomyomatosis ( DL ) .
	manualset3
128668	1	405909	13	NULL	NULL	0	NULL	intestinal obstruction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rarely they may cause intestinal obstruction , acute peritonitis due to perforation , or gastrointestinal hemorrhage .
	manualset3
128669	2	405909	13	NULL	NULL	0	NULL	acute peritonitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rarely they may cause intestinal obstruction , acute peritonitis due to perforation , or gastrointestinal hemorrhage .
	manualset3
128670	3	405909	13	NULL	NULL	0	NULL	perforation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rarely they may cause intestinal obstruction , acute peritonitis due to perforation , or gastrointestinal hemorrhage .
	manualset3
128671	4	405909	13	NULL	NULL	0	NULL	 gastrointestinal hemorrhage 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rarely they may cause intestinal obstruction , acute peritonitis due to perforation , or gastrointestinal hemorrhage .
	manualset3
128672	1	405910	13	NULL	NULL	0	NULL	method	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for the determination of cyanidin-3-glucoside ( red kernel color , RKC ) in various matrices , including carbonated soft drinks , fruit-based soft drinks , sugar confectionery and milk-based drinks , by high performance liquid chromatography ( HPLC ) based on UV-Vis detection ( at 520 nm ) have been developed .
	manualset3
128673	2	405910	13	NULL	NULL	0	NULL	determination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for the determination of cyanidin-3-glucoside ( red kernel color , RKC ) in various matrices , including carbonated soft drinks , fruit-based soft drinks , sugar confectionery and milk-based drinks , by high performance liquid chromatography ( HPLC ) based on UV-Vis detection ( at 520 nm ) have been developed .
	manualset3
128674	3	405910	13	NULL	NULL	0	NULL	cyanidin-3-glucoside 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for the determination of cyanidin-3-glucoside ( red kernel color , RKC ) in various matrices , including carbonated soft drinks , fruit-based soft drinks , sugar confectionery and milk-based drinks , by high performance liquid chromatography ( HPLC ) based on UV-Vis detection ( at 520 nm ) have been developed .
	manualset3
128675	4	405910	13	NULL	NULL	0	NULL	red kernel color , RKC	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for the determination of cyanidin-3-glucoside ( red kernel color , RKC ) in various matrices , including carbonated soft drinks , fruit-based soft drinks , sugar confectionery and milk-based drinks , by high performance liquid chromatography ( HPLC ) based on UV-Vis detection ( at 520 nm ) have been developed .
	manualset3
128676	5	405910	13	NULL	NULL	0	NULL	matrices	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for the determination of cyanidin-3-glucoside ( red kernel color , RKC ) in various matrices , including carbonated soft drinks , fruit-based soft drinks , sugar confectionery and milk-based drinks , by high performance liquid chromatography ( HPLC ) based on UV-Vis detection ( at 520 nm ) have been developed .
	manualset3
128677	6	405910	13	NULL	NULL	0	NULL	soft drinks	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for the determination of cyanidin-3-glucoside ( red kernel color , RKC ) in various matrices , including carbonated soft drinks , fruit-based soft drinks , sugar confectionery and milk-based drinks , by high performance liquid chromatography ( HPLC ) based on UV-Vis detection ( at 520 nm ) have been developed .
	manualset3
128678	7	405910	13	NULL	NULL	0	NULL	fruit-based soft drinks	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for the determination of cyanidin-3-glucoside ( red kernel color , RKC ) in various matrices , including carbonated soft drinks , fruit-based soft drinks , sugar confectionery and milk-based drinks , by high performance liquid chromatography ( HPLC ) based on UV-Vis detection ( at 520 nm ) have been developed .
	manualset3
128679	8	405910	13	NULL	NULL	0	NULL	sugar confectionery drinks 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for the determination of cyanidin-3-glucoside ( red kernel color , RKC ) in various matrices , including carbonated soft drinks , fruit-based soft drinks , sugar confectionery and milk-based drinks , by high performance liquid chromatography ( HPLC ) based on UV-Vis detection ( at 520 nm ) have been developed .
	manualset3
128680	9	405910	13	NULL	NULL	0	NULL	milk-based drinks	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for the determination of cyanidin-3-glucoside ( red kernel color , RKC ) in various matrices , including carbonated soft drinks , fruit-based soft drinks , sugar confectionery and milk-based drinks , by high performance liquid chromatography ( HPLC ) based on UV-Vis detection ( at 520 nm ) have been developed .
	manualset3
128681	10	405910	13	NULL	NULL	0	NULL	high performance liquid chromatography ( HPLC ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for the determination of cyanidin-3-glucoside ( red kernel color , RKC ) in various matrices , including carbonated soft drinks , fruit-based soft drinks , sugar confectionery and milk-based drinks , by high performance liquid chromatography ( HPLC ) based on UV-Vis detection ( at 520 nm ) have been developed .
	manualset3
128682	11	405910	13	NULL	NULL	0	NULL	UV-Vis detection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for the determination of cyanidin-3-glucoside ( red kernel color , RKC ) in various matrices , including carbonated soft drinks , fruit-based soft drinks , sugar confectionery and milk-based drinks , by high performance liquid chromatography ( HPLC ) based on UV-Vis detection ( at 520 nm ) have been developed .
	manualset3
128683	12	405910	13	NULL	NULL	0	NULL	520 nm 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for the determination of cyanidin-3-glucoside ( red kernel color , RKC ) in various matrices , including carbonated soft drinks , fruit-based soft drinks , sugar confectionery and milk-based drinks , by high performance liquid chromatography ( HPLC ) based on UV-Vis detection ( at 520 nm ) have been developed .
	manualset3
128684	1	405911	13	NULL	NULL	0	NULL	Ras	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Ras activates a multitude of downstream activities with roles in cellular processing , including invasion and metastasis .
	manualset3
128685	2	405911	13	NULL	NULL	0	NULL	multitude of downstream activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ras activates a multitude of downstream activities with roles in cellular processing , including invasion and metastasis .
	manualset3
128686	3	405911	13	NULL	NULL	0	NULL	roles 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ras activates a multitude of downstream activities with roles in cellular processing , including invasion and metastasis .
	manualset3
128687	4	405911	13	NULL	NULL	0	NULL	cellular processing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ras activates a multitude of downstream activities with roles in cellular processing , including invasion and metastasis .
	manualset3
128688	5	405911	13	NULL	NULL	0	NULL	invasion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ras activates a multitude of downstream activities with roles in cellular processing , including invasion and metastasis .
	manualset3
128689	6	405911	13	NULL	NULL	0	NULL	metastasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ras activates a multitude of downstream activities with roles in cellular processing , including invasion and metastasis .
	manualset3
128690	1	405912	13	NULL	NULL	0	NULL	Rat brain hexokinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat brain hexokinase ( ATP : D-hexose 6-phosphotransferase , EC 2.7.1.1 ) has been studied by differential scanning calorimetry .
	manualset3
128691	2	405912	13	NULL	NULL	0	NULL	ATP : D-hexose 6-phosphotransferase , EC 2.7.1.1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat brain hexokinase ( ATP : D-hexose 6-phosphotransferase , EC 2.7.1.1 ) has been studied by differential scanning calorimetry .
	manualset3
128692	3	405912	13	NULL	NULL	0	NULL	 differential scanning calorimetry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat brain hexokinase ( ATP : D-hexose 6-phosphotransferase , EC 2.7.1.1 ) has been studied by differential scanning calorimetry .
	manualset3
128693	1	405913	13	NULL	NULL	0	NULL	Rat embryos	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat embryos explanted at stages between primitive streak and head-fold were exposed in rotating bottle cultures to glucose levels raised by 3-15 mg/ml either throughout a 66-h culture period , or for shorter intervals near the start of culture ( with the rest of the culture period at normal glucose levels ) .
	manualset3
128694	2	405913	13	NULL	NULL	0	NULL	stages 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat embryos explanted at stages between primitive streak and head-fold were exposed in rotating bottle cultures to glucose levels raised by 3-15 mg/ml either throughout a 66-h culture period , or for shorter intervals near the start of culture ( with the rest of the culture period at normal glucose levels ) .
	manualset3
128695	3	405913	13	NULL	NULL	0	NULL	primitive streak	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat embryos explanted at stages between primitive streak and head-fold were exposed in rotating bottle cultures to glucose levels raised by 3-15 mg/ml either throughout a 66-h culture period , or for shorter intervals near the start of culture ( with the rest of the culture period at normal glucose levels ) .
	manualset3
128696	4	405913	13	NULL	NULL	NULL	NULL	head-fold	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Rat embryos explanted at stages between primitive streak and head-fold were exposed in rotating bottle cultures to glucose levels raised by 3-15 mg/ml either throughout a 66-h culture period , or for shorter intervals near the start of culture ( with the rest of the culture period at normal glucose levels ) .
	manualset3
128697	5	405913	13	NULL	NULL	0	NULL	rotating bottle cultures	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat embryos explanted at stages between primitive streak and head-fold were exposed in rotating bottle cultures to glucose levels raised by 3-15 mg/ml either throughout a 66-h culture period , or for shorter intervals near the start of culture ( with the rest of the culture period at normal glucose levels ) .
	manualset3
128698	6	405913	13	NULL	NULL	0	NULL	glucose levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat embryos explanted at stages between primitive streak and head-fold were exposed in rotating bottle cultures to glucose levels raised by 3-15 mg/ml either throughout a 66-h culture period , or for shorter intervals near the start of culture ( with the rest of the culture period at normal glucose levels ) .
	manualset3
128699	7	405913	13	NULL	NULL	0	NULL	3-15 mg/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat embryos explanted at stages between primitive streak and head-fold were exposed in rotating bottle cultures to glucose levels raised by 3-15 mg/ml either throughout a 66-h culture period , or for shorter intervals near the start of culture ( with the rest of the culture period at normal glucose levels ) .
	manualset3
128700	8	405913	13	NULL	NULL	0	NULL	66-h culture period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat embryos explanted at stages between primitive streak and head-fold were exposed in rotating bottle cultures to glucose levels raised by 3-15 mg/ml either throughout a 66-h culture period , or for shorter intervals near the start of culture ( with the rest of the culture period at normal glucose levels ) .
	manualset3
128701	9	405913	13	NULL	NULL	0	NULL	shorter intervals 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat embryos explanted at stages between primitive streak and head-fold were exposed in rotating bottle cultures to glucose levels raised by 3-15 mg/ml either throughout a 66-h culture period , or for shorter intervals near the start of culture ( with the rest of the culture period at normal glucose levels ) .
	manualset3
128702	10	405913	13	NULL	NULL	NULL	NULL	culture	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Rat embryos explanted at stages between primitive streak and head-fold were exposed in rotating bottle cultures to glucose levels raised by 3-15 mg/ml either throughout a 66-h culture period , or for shorter intervals near the start of culture ( with the rest of the culture period at normal glucose levels ) .
	manualset3
128703	11	405913	13	NULL	NULL	0	NULL	culture period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat embryos explanted at stages between primitive streak and head-fold were exposed in rotating bottle cultures to glucose levels raised by 3-15 mg/ml either throughout a 66-h culture period , or for shorter intervals near the start of culture ( with the rest of the culture period at normal glucose levels ) .
	manualset3
128704	12	405913	13	NULL	NULL	0	NULL	normal glucose levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat embryos explanted at stages between primitive streak and head-fold were exposed in rotating bottle cultures to glucose levels raised by 3-15 mg/ml either throughout a 66-h culture period , or for shorter intervals near the start of culture ( with the rest of the culture period at normal glucose levels ) .
	manualset3
128705	1	405914	13	NULL	NULL	0	NULL	Rat glomeruli 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat glomeruli and papillae possess the enzymes necessary to process leukotriene C4 into leukotrienes D4 and E4 .
	manualset3
128706	2	405914	13	NULL	NULL	0	NULL	papillae	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat glomeruli and papillae possess the enzymes necessary to process leukotriene C4 into leukotrienes D4 and E4 .
	manualset3
128707	3	405914	13	NULL	NULL	0	NULL	enzymes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat glomeruli and papillae possess the enzymes necessary to process leukotriene C4 into leukotrienes D4 and E4 .
	manualset3
128708	4	405914	13	NULL	NULL	0	NULL	leukotriene C4 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat glomeruli and papillae possess the enzymes necessary to process leukotriene C4 into leukotrienes D4 and E4 .
	manualset3
128709	5	405914	13	NULL	NULL	0	NULL	leukotrienes D4	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat glomeruli and papillae possess the enzymes necessary to process leukotriene C4 into leukotrienes D4 and E4 .
	manualset3
128710	6	405914	13	NULL	NULL	0	NULL	leukotrienes E4 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat glomeruli and papillae possess the enzymes necessary to process leukotriene C4 into leukotrienes D4 and E4 .
	manualset3
128711	1	405915	13	NULL	NULL	0	NULL	Rat hypoplastic kidney ( hpk/hpk )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat hypoplastic kidney ( hpk/hpk ) induces renal anemia , hyperparathyroidism , and osteodystrophy at the end stage of renal failure .
	manualset3
128712	2	405915	13	NULL	NULL	0	NULL	renal anemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat hypoplastic kidney ( hpk/hpk ) induces renal anemia , hyperparathyroidism , and osteodystrophy at the end stage of renal failure .
	manualset3
128713	3	405915	13	NULL	NULL	0	NULL	hyperparathyroidism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat hypoplastic kidney ( hpk/hpk ) induces renal anemia , hyperparathyroidism , and osteodystrophy at the end stage of renal failure .
	manualset3
128714	4	405915	13	NULL	NULL	0	NULL	osteodystrophy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat hypoplastic kidney ( hpk/hpk ) induces renal anemia , hyperparathyroidism , and osteodystrophy at the end stage of renal failure .
	manualset3
128715	5	405915	13	NULL	NULL	0	NULL	end stage of renal failure 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat hypoplastic kidney ( hpk/hpk ) induces renal anemia , hyperparathyroidism , and osteodystrophy at the end stage of renal failure .
	manualset3
128716	1	405916	13	NULL	NULL	0	NULL	Rat islets 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat islets treated with a cytokine combination ( interleukin ( IL ) -1 beta , tumor necrosis factor ( TNF ) - alpha and interferon ( IFN ) - gamma ) displayed a significant increase in islet cell apoptosis when the islets were incubated in 24.4 mM glucose compared with untreated islets at the same glucose concentration ( 13.07 + / - 1.78 % vs 6.09 + / - 0.78 % ; P & lt ; 0.01 ) or islets incubated in 5.5 mM glucose concentration and cytokines ( 13.07 + / - 1.78 % vs 8.04 + / - 1.56 % ; P & lt ; 0.05 ) .
	manualset3
128717	2	405916	13	NULL	NULL	0	NULL	cytokine combination	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat islets treated with a cytokine combination ( interleukin ( IL ) -1 beta , tumor necrosis factor ( TNF ) - alpha and interferon ( IFN ) - gamma ) displayed a significant increase in islet cell apoptosis when the islets were incubated in 24.4 mM glucose compared with untreated islets at the same glucose concentration ( 13.07 + / - 1.78 % vs 6.09 + / - 0.78 % ; P & lt ; 0.01 ) or islets incubated in 5.5 mM glucose concentration and cytokines ( 13.07 + / - 1.78 % vs 8.04 + / - 1.56 % ; P & lt ; 0.05 ) .
	manualset3
128718	3	405916	13	NULL	NULL	0	NULL	 interleukin ( IL ) -1 beta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat islets treated with a cytokine combination ( interleukin ( IL ) -1 beta , tumor necrosis factor ( TNF ) - alpha and interferon ( IFN ) - gamma ) displayed a significant increase in islet cell apoptosis when the islets were incubated in 24.4 mM glucose compared with untreated islets at the same glucose concentration ( 13.07 + / - 1.78 % vs 6.09 + / - 0.78 % ; P & lt ; 0.01 ) or islets incubated in 5.5 mM glucose concentration and cytokines ( 13.07 + / - 1.78 % vs 8.04 + / - 1.56 % ; P & lt ; 0.05 ) .
	manualset3
128719	4	405916	13	NULL	NULL	0	NULL	tumor necrosis factor ( TNF ) - alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat islets treated with a cytokine combination ( interleukin ( IL ) -1 beta , tumor necrosis factor ( TNF ) - alpha and interferon ( IFN ) - gamma ) displayed a significant increase in islet cell apoptosis when the islets were incubated in 24.4 mM glucose compared with untreated islets at the same glucose concentration ( 13.07 + / - 1.78 % vs 6.09 + / - 0.78 % ; P & lt ; 0.01 ) or islets incubated in 5.5 mM glucose concentration and cytokines ( 13.07 + / - 1.78 % vs 8.04 + / - 1.56 % ; P & lt ; 0.05 ) .
	manualset3
128720	5	405916	13	NULL	NULL	0	NULL	interferon ( IFN ) - gamma	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat islets treated with a cytokine combination ( interleukin ( IL ) -1 beta , tumor necrosis factor ( TNF ) - alpha and interferon ( IFN ) - gamma ) displayed a significant increase in islet cell apoptosis when the islets were incubated in 24.4 mM glucose compared with untreated islets at the same glucose concentration ( 13.07 + / - 1.78 % vs 6.09 + / - 0.78 % ; P & lt ; 0.01 ) or islets incubated in 5.5 mM glucose concentration and cytokines ( 13.07 + / - 1.78 % vs 8.04 + / - 1.56 % ; P & lt ; 0.05 ) .
	manualset3
128721	6	405916	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat islets treated with a cytokine combination ( interleukin ( IL ) -1 beta , tumor necrosis factor ( TNF ) - alpha and interferon ( IFN ) - gamma ) displayed a significant increase in islet cell apoptosis when the islets were incubated in 24.4 mM glucose compared with untreated islets at the same glucose concentration ( 13.07 + / - 1.78 % vs 6.09 + / - 0.78 % ; P & lt ; 0.01 ) or islets incubated in 5.5 mM glucose concentration and cytokines ( 13.07 + / - 1.78 % vs 8.04 + / - 1.56 % ; P & lt ; 0.05 ) .
	manualset3
128722	7	405916	13	NULL	NULL	0	NULL	islet cell apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat islets treated with a cytokine combination ( interleukin ( IL ) -1 beta , tumor necrosis factor ( TNF ) - alpha and interferon ( IFN ) - gamma ) displayed a significant increase in islet cell apoptosis when the islets were incubated in 24.4 mM glucose compared with untreated islets at the same glucose concentration ( 13.07 + / - 1.78 % vs 6.09 + / - 0.78 % ; P & lt ; 0.01 ) or islets incubated in 5.5 mM glucose concentration and cytokines ( 13.07 + / - 1.78 % vs 8.04 + / - 1.56 % ; P & lt ; 0.05 ) .
	manualset3
128723	8	405916	13	NULL	NULL	0	NULL	 islets 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat islets treated with a cytokine combination ( interleukin ( IL ) -1 beta , tumor necrosis factor ( TNF ) - alpha and interferon ( IFN ) - gamma ) displayed a significant increase in islet cell apoptosis when the islets were incubated in 24.4 mM glucose compared with untreated islets at the same glucose concentration ( 13.07 + / - 1.78 % vs 6.09 + / - 0.78 % ; P & lt ; 0.01 ) or islets incubated in 5.5 mM glucose concentration and cytokines ( 13.07 + / - 1.78 % vs 8.04 + / - 1.56 % ; P & lt ; 0.05 ) .
	manualset3
128724	9	405916	13	NULL	NULL	0	NULL	24.4 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat islets treated with a cytokine combination ( interleukin ( IL ) -1 beta , tumor necrosis factor ( TNF ) - alpha and interferon ( IFN ) - gamma ) displayed a significant increase in islet cell apoptosis when the islets were incubated in 24.4 mM glucose compared with untreated islets at the same glucose concentration ( 13.07 + / - 1.78 % vs 6.09 + / - 0.78 % ; P & lt ; 0.01 ) or islets incubated in 5.5 mM glucose concentration and cytokines ( 13.07 + / - 1.78 % vs 8.04 + / - 1.56 % ; P & lt ; 0.05 ) .
	manualset3
128725	10	405916	13	NULL	NULL	0	NULL	glucose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat islets treated with a cytokine combination ( interleukin ( IL ) -1 beta , tumor necrosis factor ( TNF ) - alpha and interferon ( IFN ) - gamma ) displayed a significant increase in islet cell apoptosis when the islets were incubated in 24.4 mM glucose compared with untreated islets at the same glucose concentration ( 13.07 + / - 1.78 % vs 6.09 + / - 0.78 % ; P & lt ; 0.01 ) or islets incubated in 5.5 mM glucose concentration and cytokines ( 13.07 + / - 1.78 % vs 8.04 + / - 1.56 % ; P & lt ; 0.05 ) .
	manualset3
128727	11	405916	13	NULL	NULL	0	NULL	islets	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat islets treated with a cytokine combination ( interleukin ( IL ) -1 beta , tumor necrosis factor ( TNF ) - alpha and interferon ( IFN ) - gamma ) displayed a significant increase in islet cell apoptosis when the islets were incubated in 24.4 mM glucose compared with untreated islets at the same glucose concentration ( 13.07 + / - 1.78 % vs 6.09 + / - 0.78 % ; P & lt ; 0.01 ) or islets incubated in 5.5 mM glucose concentration and cytokines ( 13.07 + / - 1.78 % vs 8.04 + / - 1.56 % ; P & lt ; 0.05 ) .
	manualset3
128728	12	405916	13	NULL	NULL	0	NULL	glucose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat islets treated with a cytokine combination ( interleukin ( IL ) -1 beta , tumor necrosis factor ( TNF ) - alpha and interferon ( IFN ) - gamma ) displayed a significant increase in islet cell apoptosis when the islets were incubated in 24.4 mM glucose compared with untreated islets at the same glucose concentration ( 13.07 + / - 1.78 % vs 6.09 + / - 0.78 % ; P & lt ; 0.01 ) or islets incubated in 5.5 mM glucose concentration and cytokines ( 13.07 + / - 1.78 % vs 8.04 + / - 1.56 % ; P & lt ; 0.05 ) .
	manualset3
128729	13	405916	13	NULL	NULL	0	NULL	concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat islets treated with a cytokine combination ( interleukin ( IL ) -1 beta , tumor necrosis factor ( TNF ) - alpha and interferon ( IFN ) - gamma ) displayed a significant increase in islet cell apoptosis when the islets were incubated in 24.4 mM glucose compared with untreated islets at the same glucose concentration ( 13.07 + / - 1.78 % vs 6.09 + / - 0.78 % ; P & lt ; 0.01 ) or islets incubated in 5.5 mM glucose concentration and cytokines ( 13.07 + / - 1.78 % vs 8.04 + / - 1.56 % ; P & lt ; 0.05 ) .
	manualset3
128730	14	405916	13	NULL	NULL	0	NULL	13.07 + / - 1.78 % vs 6.09 + / - 0.78 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat islets treated with a cytokine combination ( interleukin ( IL ) -1 beta , tumor necrosis factor ( TNF ) - alpha and interferon ( IFN ) - gamma ) displayed a significant increase in islet cell apoptosis when the islets were incubated in 24.4 mM glucose compared with untreated islets at the same glucose concentration ( 13.07 + / - 1.78 % vs 6.09 + / - 0.78 % ; P & lt ; 0.01 ) or islets incubated in 5.5 mM glucose concentration and cytokines ( 13.07 + / - 1.78 % vs 8.04 + / - 1.56 % ; P & lt ; 0.05 ) .
	manualset3
128731	15	405916	13	NULL	NULL	0	NULL	P & lt ; 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat islets treated with a cytokine combination ( interleukin ( IL ) -1 beta , tumor necrosis factor ( TNF ) - alpha and interferon ( IFN ) - gamma ) displayed a significant increase in islet cell apoptosis when the islets were incubated in 24.4 mM glucose compared with untreated islets at the same glucose concentration ( 13.07 + / - 1.78 % vs 6.09 + / - 0.78 % ; P & lt ; 0.01 ) or islets incubated in 5.5 mM glucose concentration and cytokines ( 13.07 + / - 1.78 % vs 8.04 + / - 1.56 % ; P & lt ; 0.05 ) .
	manualset3
128732	16	405916	13	NULL	NULL	0	NULL	islets	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat islets treated with a cytokine combination ( interleukin ( IL ) -1 beta , tumor necrosis factor ( TNF ) - alpha and interferon ( IFN ) - gamma ) displayed a significant increase in islet cell apoptosis when the islets were incubated in 24.4 mM glucose compared with untreated islets at the same glucose concentration ( 13.07 + / - 1.78 % vs 6.09 + / - 0.78 % ; P & lt ; 0.01 ) or islets incubated in 5.5 mM glucose concentration and cytokines ( 13.07 + / - 1.78 % vs 8.04 + / - 1.56 % ; P & lt ; 0.05 ) .
	manualset3
128733	17	405916	13	NULL	NULL	0	NULL	5.5 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat islets treated with a cytokine combination ( interleukin ( IL ) -1 beta , tumor necrosis factor ( TNF ) - alpha and interferon ( IFN ) - gamma ) displayed a significant increase in islet cell apoptosis when the islets were incubated in 24.4 mM glucose compared with untreated islets at the same glucose concentration ( 13.07 + / - 1.78 % vs 6.09 + / - 0.78 % ; P & lt ; 0.01 ) or islets incubated in 5.5 mM glucose concentration and cytokines ( 13.07 + / - 1.78 % vs 8.04 + / - 1.56 % ; P & lt ; 0.05 ) .
	manualset3
128734	18	405916	13	NULL	NULL	0	NULL	glucose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat islets treated with a cytokine combination ( interleukin ( IL ) -1 beta , tumor necrosis factor ( TNF ) - alpha and interferon ( IFN ) - gamma ) displayed a significant increase in islet cell apoptosis when the islets were incubated in 24.4 mM glucose compared with untreated islets at the same glucose concentration ( 13.07 + / - 1.78 % vs 6.09 + / - 0.78 % ; P & lt ; 0.01 ) or islets incubated in 5.5 mM glucose concentration and cytokines ( 13.07 + / - 1.78 % vs 8.04 + / - 1.56 % ; P & lt ; 0.05 ) .
	manualset3
128735	19	405916	13	NULL	NULL	0	NULL	concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat islets treated with a cytokine combination ( interleukin ( IL ) -1 beta , tumor necrosis factor ( TNF ) - alpha and interferon ( IFN ) - gamma ) displayed a significant increase in islet cell apoptosis when the islets were incubated in 24.4 mM glucose compared with untreated islets at the same glucose concentration ( 13.07 + / - 1.78 % vs 6.09 + / - 0.78 % ; P & lt ; 0.01 ) or islets incubated in 5.5 mM glucose concentration and cytokines ( 13.07 + / - 1.78 % vs 8.04 + / - 1.56 % ; P & lt ; 0.05 ) .
	manualset3
128736	20	405916	13	NULL	NULL	0	NULL	cytokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat islets treated with a cytokine combination ( interleukin ( IL ) -1 beta , tumor necrosis factor ( TNF ) - alpha and interferon ( IFN ) - gamma ) displayed a significant increase in islet cell apoptosis when the islets were incubated in 24.4 mM glucose compared with untreated islets at the same glucose concentration ( 13.07 + / - 1.78 % vs 6.09 + / - 0.78 % ; P & lt ; 0.01 ) or islets incubated in 5.5 mM glucose concentration and cytokines ( 13.07 + / - 1.78 % vs 8.04 + / - 1.56 % ; P & lt ; 0.05 ) .
	manualset3
128737	21	405916	13	NULL	NULL	0	NULL	13.07 + / - 1.78 % vs 8.04 + / - 1.56 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat islets treated with a cytokine combination ( interleukin ( IL ) -1 beta , tumor necrosis factor ( TNF ) - alpha and interferon ( IFN ) - gamma ) displayed a significant increase in islet cell apoptosis when the islets were incubated in 24.4 mM glucose compared with untreated islets at the same glucose concentration ( 13.07 + / - 1.78 % vs 6.09 + / - 0.78 % ; P & lt ; 0.01 ) or islets incubated in 5.5 mM glucose concentration and cytokines ( 13.07 + / - 1.78 % vs 8.04 + / - 1.56 % ; P & lt ; 0.05 ) .
	manualset3
128738	22	405916	13	NULL	NULL	0	NULL	P & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat islets treated with a cytokine combination ( interleukin ( IL ) -1 beta , tumor necrosis factor ( TNF ) - alpha and interferon ( IFN ) - gamma ) displayed a significant increase in islet cell apoptosis when the islets were incubated in 24.4 mM glucose compared with untreated islets at the same glucose concentration ( 13.07 + / - 1.78 % vs 6.09 + / - 0.78 % ; P & lt ; 0.01 ) or islets incubated in 5.5 mM glucose concentration and cytokines ( 13.07 + / - 1.78 % vs 8.04 + / - 1.56 % ; P & lt ; 0.05 ) .
	manualset3
128739	1	405917	13	NULL	NULL	0	NULL	Rat liver survival 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat liver survival after 14 hours of preservation was higher in low-K + solutions ( 13 of 13 ) than in high-K + solutions ( 7 of 13 ) .
	manualset3
128740	2	405917	13	NULL	NULL	0	NULL	14 hours	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat liver survival after 14 hours of preservation was higher in low-K + solutions ( 13 of 13 ) than in high-K + solutions ( 7 of 13 ) .
	manualset3
128741	3	405917	13	NULL	NULL	0	NULL	preservation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat liver survival after 14 hours of preservation was higher in low-K + solutions ( 13 of 13 ) than in high-K + solutions ( 7 of 13 ) .
	manualset3
128742	4	405917	13	NULL	NULL	0	NULL	low-K + solutions 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat liver survival after 14 hours of preservation was higher in low-K + solutions ( 13 of 13 ) than in high-K + solutions ( 7 of 13 ) .
	manualset3
128743	5	405917	13	NULL	NULL	0	NULL	13 of 13 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat liver survival after 14 hours of preservation was higher in low-K + solutions ( 13 of 13 ) than in high-K + solutions ( 7 of 13 ) .
	manualset3
128744	6	405917	13	NULL	NULL	0	NULL	high-K + solutions 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat liver survival after 14 hours of preservation was higher in low-K + solutions ( 13 of 13 ) than in high-K + solutions ( 7 of 13 ) .
	manualset3
128745	7	405917	13	NULL	NULL	0	NULL	7 of 13	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rat liver survival after 14 hours of preservation was higher in low-K + solutions ( 13 of 13 ) than in high-K + solutions ( 7 of 13 ) .
	manualset3
128746	1	405918	13	NULL	NULL	0	NULL	Rate of bone loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rate of bone loss in postmenopausal and osteoporotic women .
	manualset3
128747	2	405918	13	NULL	NULL	0	NULL	postmenopausal women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Rate of bone loss in postmenopausal and osteoporotic women .
	manualset3
128748	3	405918	13	NULL	NULL	0	NULL	osteoporotic women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Rate of bone loss in postmenopausal and osteoporotic women .
	manualset3
128749	1	405919	13	NULL	NULL	0	NULL	Rate of drainage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rate of drainage of the blood vessels of the limbs by gravity .
	manualset3
128750	2	405919	13	NULL	NULL	0	NULL	blood vessels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Rate of drainage of the blood vessels of the limbs by gravity .
	manualset3
128751	3	405919	13	NULL	NULL	0	NULL	limbs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Rate of drainage of the blood vessels of the limbs by gravity .
	manualset3
128752	4	405919	13	NULL	NULL	0	NULL	gravity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rate of drainage of the blood vessels of the limbs by gravity .
	manualset3
128753	1	405920	13	NULL	NULL	0	NULL	method	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for the improvement of human sperm motility in vitro .
	manualset3
128754	2	405920	13	NULL	NULL	0	NULL	improvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for the improvement of human sperm motility in vitro .
	manualset3
128755	3	405920	13	NULL	NULL	0	NULL	human sperm motility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for the improvement of human sperm motility in vitro .
	manualset3
128756	1	405921	13	NULL	NULL	0	NULL	Rates 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rates of disappearance from plasma of enzymes labeled by coupling with a radioactive lodo-ester .
	manualset3
128757	2	405921	13	NULL	NULL	0	NULL	disappearance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rates of disappearance from plasma of enzymes labeled by coupling with a radioactive lodo-ester .
	manualset3
128758	3	405921	13	NULL	NULL	0	NULL	plasma of enzymes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Rates of disappearance from plasma of enzymes labeled by coupling with a radioactive lodo-ester .
	manualset3
128759	4	405921	13	NULL	NULL	0	NULL	radioactive lodo-ester	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rates of disappearance from plasma of enzymes labeled by coupling with a radioactive lodo-ester .
	manualset3
128760	1	405922	13	NULL	NULL	0	NULL	Rates	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rates of glycogen synthase ( V ( syn ) ) and phosphorylase ( V ( phos ) ) flux were estimated during a ( 1 - ( 13 ) C ) glucose ( pulse ) - unlabeled glucose ( chase ) infusion .
	manualset3
128761	2	405922	13	NULL	NULL	0	NULL	glycogen synthase ( V ( syn ) ) flux 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rates of glycogen synthase ( V ( syn ) ) and phosphorylase ( V ( phos ) ) flux were estimated during a ( 1 - ( 13 ) C ) glucose ( pulse ) - unlabeled glucose ( chase ) infusion .
	manualset3
128762	3	405922	13	NULL	NULL	0	NULL	phosphorylase ( V ( phos ) ) flux 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rates of glycogen synthase ( V ( syn ) ) and phosphorylase ( V ( phos ) ) flux were estimated during a ( 1 - ( 13 ) C ) glucose ( pulse ) - unlabeled glucose ( chase ) infusion .
	manualset3
128763	4	405922	13	NULL	NULL	0	NULL	( 1 - ( 13 ) C ) glucose ( pulse ) - unlabeled glucose ( chase ) infusion 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rates of glycogen synthase ( V ( syn ) ) and phosphorylase ( V ( phos ) ) flux were estimated during a ( 1 - ( 13 ) C ) glucose ( pulse ) - unlabeled glucose ( chase ) infusion .
	manualset3
128764	1	405923	13	NULL	NULL	0	NULL	Rates	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rates of prior victimization were very high with 71 % of women reporting a childhood experience of physical abuse and 53 % of women reporting a childhood experience of sexual abuse .
	manualset3
128765	2	405923	13	NULL	NULL	0	NULL	victimization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rates of prior victimization were very high with 71 % of women reporting a childhood experience of physical abuse and 53 % of women reporting a childhood experience of sexual abuse .
	manualset3
128766	3	405923	13	NULL	NULL	0	NULL	71 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rates of prior victimization were very high with 71 % of women reporting a childhood experience of physical abuse and 53 % of women reporting a childhood experience of sexual abuse .
	manualset3
128767	4	405923	13	NULL	NULL	0	NULL	women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Rates of prior victimization were very high with 71 % of women reporting a childhood experience of physical abuse and 53 % of women reporting a childhood experience of sexual abuse .
	manualset3
128768	5	405923	13	NULL	NULL	0	NULL	childhood experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rates of prior victimization were very high with 71 % of women reporting a childhood experience of physical abuse and 53 % of women reporting a childhood experience of sexual abuse .
	manualset3
128769	6	405923	13	NULL	NULL	NULL	NULL	physical abuse 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Rates of prior victimization were very high with 71 % of women reporting a childhood experience of physical abuse and 53 % of women reporting a childhood experience of sexual abuse .
	manualset3
128770	7	405923	13	NULL	NULL	0	NULL	53 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rates of prior victimization were very high with 71 % of women reporting a childhood experience of physical abuse and 53 % of women reporting a childhood experience of sexual abuse .
	manualset3
128771	8	405923	13	NULL	NULL	0	NULL	women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Rates of prior victimization were very high with 71 % of women reporting a childhood experience of physical abuse and 53 % of women reporting a childhood experience of sexual abuse .
	manualset3
128772	9	405923	13	NULL	NULL	0	NULL	childhood experience 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rates of prior victimization were very high with 71 % of women reporting a childhood experience of physical abuse and 53 % of women reporting a childhood experience of sexual abuse .
	manualset3
128773	10	405923	13	NULL	NULL	0	NULL	sexual abuse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rates of prior victimization were very high with 71 % of women reporting a childhood experience of physical abuse and 53 % of women reporting a childhood experience of sexual abuse .
	manualset3
128774	1	405924	13	NULL	NULL	0	NULL	cooperativity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather , the apparent cooperativity observed in protein kinase C 's interaction with multiple phosphatidylserine molecules arises from effects specific to the interaction of a multivalent macromolecule with multiple membrane-associated ligands .
	manualset3
128775	2	405924	13	NULL	NULL	0	NULL	protein kinase C 's 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather , the apparent cooperativity observed in protein kinase C 's interaction with multiple phosphatidylserine molecules arises from effects specific to the interaction of a multivalent macromolecule with multiple membrane-associated ligands .
	manualset3
128776	3	405924	13	NULL	NULL	0	NULL	interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather , the apparent cooperativity observed in protein kinase C 's interaction with multiple phosphatidylserine molecules arises from effects specific to the interaction of a multivalent macromolecule with multiple membrane-associated ligands .
	manualset3
128777	4	405924	13	NULL	NULL	0	NULL	multiple phosphatidylserine molecules	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather , the apparent cooperativity observed in protein kinase C 's interaction with multiple phosphatidylserine molecules arises from effects specific to the interaction of a multivalent macromolecule with multiple membrane-associated ligands .
	manualset3
128778	5	405924	13	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather , the apparent cooperativity observed in protein kinase C 's interaction with multiple phosphatidylserine molecules arises from effects specific to the interaction of a multivalent macromolecule with multiple membrane-associated ligands .
	manualset3
128779	6	405924	13	NULL	NULL	0	NULL	interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather , the apparent cooperativity observed in protein kinase C 's interaction with multiple phosphatidylserine molecules arises from effects specific to the interaction of a multivalent macromolecule with multiple membrane-associated ligands .
	manualset3
128780	7	405924	13	NULL	NULL	0	NULL	multivalent macromolecule	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather , the apparent cooperativity observed in protein kinase C 's interaction with multiple phosphatidylserine molecules arises from effects specific to the interaction of a multivalent macromolecule with multiple membrane-associated ligands .
	manualset3
128781	8	405924	13	NULL	NULL	0	NULL	multiple membrane-associated ligands	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather , the apparent cooperativity observed in protein kinase C 's interaction with multiple phosphatidylserine molecules arises from effects specific to the interaction of a multivalent macromolecule with multiple membrane-associated ligands .
	manualset3
128782	1	405925	13	NULL	NULL	0	NULL	effects 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather , the effects of lipopolysaccharide involved the production of inflammatory cytokines , in particular TNF alpha .
	manualset3
128783	2	405925	13	NULL	NULL	0	NULL	lipopolysaccharide	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather , the effects of lipopolysaccharide involved the production of inflammatory cytokines , in particular TNF alpha .
	manualset3
128784	3	405925	13	NULL	NULL	0	NULL	production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather , the effects of lipopolysaccharide involved the production of inflammatory cytokines , in particular TNF alpha .
	manualset3
128785	4	405925	13	NULL	NULL	0	NULL	inflammatory cytokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather , the effects of lipopolysaccharide involved the production of inflammatory cytokines , in particular TNF alpha .
	manualset3
128786	5	405925	13	NULL	NULL	0	NULL	TNF alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather , the effects of lipopolysaccharide involved the production of inflammatory cytokines , in particular TNF alpha .
	manualset3
128787	1	405926	13	NULL	NULL	0	NULL	Parkinson 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather it appears that Parkinson 's disease affects several classes of neurons in localized areas of the brainstem .
	manualset3
128788	2	405926	13	NULL	NULL	0	NULL	several classes of neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather it appears that Parkinson 's disease affects several classes of neurons in localized areas of the brainstem .
	manualset3
128789	3	405926	13	NULL	NULL	0	NULL	localized areas 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather it appears that Parkinson 's disease affects several classes of neurons in localized areas of the brainstem .
	manualset3
128790	4	405926	13	NULL	NULL	0	NULL	brainstem 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather it appears that Parkinson 's disease affects several classes of neurons in localized areas of the brainstem .
	manualset3
128791	1	405927	13	NULL	NULL	0	NULL	culture	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather than bound to one culture , fallen fontanelle has been labeled as an illness or recognized as a symptom through time and space .
	manualset3
128792	2	405927	13	NULL	NULL	0	NULL	fallen fontanelle 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather than bound to one culture , fallen fontanelle has been labeled as an illness or recognized as a symptom through time and space .
	manualset3
128793	3	405927	13	NULL	NULL	0	NULL	illness 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather than bound to one culture , fallen fontanelle has been labeled as an illness or recognized as a symptom through time and space .
	manualset3
128794	4	405927	13	NULL	NULL	0	NULL	symptom 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather than bound to one culture , fallen fontanelle has been labeled as an illness or recognized as a symptom through time and space .
	manualset3
128795	5	405927	13	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather than bound to one culture , fallen fontanelle has been labeled as an illness or recognized as a symptom through time and space .
	manualset3
128796	6	405927	13	NULL	NULL	0	NULL	space	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather than bound to one culture , fallen fontanelle has been labeled as an illness or recognized as a symptom through time and space .
	manualset3
128797	1	405928	13	NULL	NULL	0	NULL	discrete changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather than discrete changes , Massachusetts has responded to these emerging trends with a new and comprehensive initiative that emphasizes one set of statewide standards in these emerging content areas for all residency training programs .
	manualset3
128798	2	405928	13	NULL	NULL	0	NULL	Massachusetts 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather than discrete changes , Massachusetts has responded to these emerging trends with a new and comprehensive initiative that emphasizes one set of statewide standards in these emerging content areas for all residency training programs .
	manualset3
128799	3	405928	13	NULL	NULL	0	NULL	trends	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather than discrete changes , Massachusetts has responded to these emerging trends with a new and comprehensive initiative that emphasizes one set of statewide standards in these emerging content areas for all residency training programs .
	manualset3
128800	4	405928	13	NULL	NULL	0	NULL	comprehensive initiative	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather than discrete changes , Massachusetts has responded to these emerging trends with a new and comprehensive initiative that emphasizes one set of statewide standards in these emerging content areas for all residency training programs .
	manualset3
128801	5	405928	13	NULL	NULL	0	NULL	set of statewide standards	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather than discrete changes , Massachusetts has responded to these emerging trends with a new and comprehensive initiative that emphasizes one set of statewide standards in these emerging content areas for all residency training programs .
	manualset3
128802	6	405928	13	NULL	NULL	0	NULL	content areas	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather than discrete changes , Massachusetts has responded to these emerging trends with a new and comprehensive initiative that emphasizes one set of statewide standards in these emerging content areas for all residency training programs .
	manualset3
128803	7	405928	13	NULL	NULL	0	NULL	residency training programs	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather than discrete changes , Massachusetts has responded to these emerging trends with a new and comprehensive initiative that emphasizes one set of statewide standards in these emerging content areas for all residency training programs .
	manualset3
128804	1	405929	13	NULL	NULL	0	NULL	Rationale 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rationale for the combination therapy of 5FU and CDDP .
	manualset3
128805	2	405929	13	NULL	NULL	0	NULL	combination therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Rationale for the combination therapy of 5FU and CDDP .
	manualset3
128806	3	405929	13	NULL	NULL	0	NULL	5FU	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Rationale for the combination therapy of 5FU and CDDP .
	manualset3
129239	4	405929	13	NULL	NULL	NULL	NULL	CDDP	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Rationale for the combination therapy of 5FU and CDDP .
	manualset3
129240	1	405930	13	NULL	NULL	0	NULL	Rationale	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rationale for use of platelet-suppressive drugs .
	manualset3
129241	2	405930	13	NULL	NULL	0	NULL	platelet-suppressive drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Rationale for use of platelet-suppressive drugs .
	manualset3
131917	3	405930	13	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rationale for use of platelet-suppressive drugs .
	manualset3
129242	1	405931	13	NULL	NULL	0	NULL	biotransformation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rationally engineered biotransformation of p-nitrophenol .
	manualset3
129243	2	405931	13	NULL	NULL	0	NULL	p-nitrophenol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rationally engineered biotransformation of p-nitrophenol .
	manualset3
129244	1	405932	13	NULL	NULL	0	NULL	Ratios	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ratios and statistically insignificant data were not used to emphasize ICD benefits .
	manualset3
129245	2	405932	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Ratios and statistically insignificant data were not used to emphasize ICD benefits .
	manualset3
129246	3	405932	13	NULL	NULL	0	NULL	ICD benefits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ratios and statistically insignificant data were not used to emphasize ICD benefits .
	manualset3
129247	1	405933	13	NULL	NULL	0	NULL	Rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats and dogs were also dosed iv for 91 days ( 3 injections/week ) with 4 ' - epidoxorubicin or doxorubicin at doses of 0.128 , 0.32 , and 0.8 mg/kg to rats and 0.064 , 0.16 , and 0.4 mg/kg to dogs .
	manualset3
129248	2	405933	13	NULL	NULL	0	NULL	dogs 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats and dogs were also dosed iv for 91 days ( 3 injections/week ) with 4 ' - epidoxorubicin or doxorubicin at doses of 0.128 , 0.32 , and 0.8 mg/kg to rats and 0.064 , 0.16 , and 0.4 mg/kg to dogs .
	manualset3
129249	3	405933	13	NULL	NULL	0	NULL	iv	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats and dogs were also dosed iv for 91 days ( 3 injections/week ) with 4 ' - epidoxorubicin or doxorubicin at doses of 0.128 , 0.32 , and 0.8 mg/kg to rats and 0.064 , 0.16 , and 0.4 mg/kg to dogs .
	manualset3
129250	4	405933	13	NULL	NULL	0	NULL	91 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats and dogs were also dosed iv for 91 days ( 3 injections/week ) with 4 ' - epidoxorubicin or doxorubicin at doses of 0.128 , 0.32 , and 0.8 mg/kg to rats and 0.064 , 0.16 , and 0.4 mg/kg to dogs .
	manualset3
129251	5	405933	13	NULL	NULL	0	NULL	3 injections/week	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats and dogs were also dosed iv for 91 days ( 3 injections/week ) with 4 ' - epidoxorubicin or doxorubicin at doses of 0.128 , 0.32 , and 0.8 mg/kg to rats and 0.064 , 0.16 , and 0.4 mg/kg to dogs .
	manualset3
129252	6	405933	13	NULL	NULL	0	NULL	4 ' - epidoxorubicin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats and dogs were also dosed iv for 91 days ( 3 injections/week ) with 4 ' - epidoxorubicin or doxorubicin at doses of 0.128 , 0.32 , and 0.8 mg/kg to rats and 0.064 , 0.16 , and 0.4 mg/kg to dogs .
	manualset3
129253	7	405933	13	NULL	NULL	0	NULL	doxorubicin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats and dogs were also dosed iv for 91 days ( 3 injections/week ) with 4 ' - epidoxorubicin or doxorubicin at doses of 0.128 , 0.32 , and 0.8 mg/kg to rats and 0.064 , 0.16 , and 0.4 mg/kg to dogs .
	manualset3
129254	8	405933	13	NULL	NULL	0	NULL	doses 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats and dogs were also dosed iv for 91 days ( 3 injections/week ) with 4 ' - epidoxorubicin or doxorubicin at doses of 0.128 , 0.32 , and 0.8 mg/kg to rats and 0.064 , 0.16 , and 0.4 mg/kg to dogs .
	manualset3
129255	9	405933	13	NULL	NULL	0	NULL	0.128 mg/kg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats and dogs were also dosed iv for 91 days ( 3 injections/week ) with 4 ' - epidoxorubicin or doxorubicin at doses of 0.128 , 0.32 , and 0.8 mg/kg to rats and 0.064 , 0.16 , and 0.4 mg/kg to dogs .
	manualset3
129256	10	405933	13	NULL	NULL	0	NULL	0.32 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats and dogs were also dosed iv for 91 days ( 3 injections/week ) with 4 ' - epidoxorubicin or doxorubicin at doses of 0.128 , 0.32 , and 0.8 mg/kg to rats and 0.064 , 0.16 , and 0.4 mg/kg to dogs .
	manualset3
129257	11	405933	13	NULL	NULL	0	NULL	0.8 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats and dogs were also dosed iv for 91 days ( 3 injections/week ) with 4 ' - epidoxorubicin or doxorubicin at doses of 0.128 , 0.32 , and 0.8 mg/kg to rats and 0.064 , 0.16 , and 0.4 mg/kg to dogs .
	manualset3
129258	12	405933	13	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats and dogs were also dosed iv for 91 days ( 3 injections/week ) with 4 ' - epidoxorubicin or doxorubicin at doses of 0.128 , 0.32 , and 0.8 mg/kg to rats and 0.064 , 0.16 , and 0.4 mg/kg to dogs .
	manualset3
129259	13	405933	13	NULL	NULL	0	NULL	0.064 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats and dogs were also dosed iv for 91 days ( 3 injections/week ) with 4 ' - epidoxorubicin or doxorubicin at doses of 0.128 , 0.32 , and 0.8 mg/kg to rats and 0.064 , 0.16 , and 0.4 mg/kg to dogs .
	manualset3
129260	14	405933	13	NULL	NULL	0	NULL	0.16 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats and dogs were also dosed iv for 91 days ( 3 injections/week ) with 4 ' - epidoxorubicin or doxorubicin at doses of 0.128 , 0.32 , and 0.8 mg/kg to rats and 0.064 , 0.16 , and 0.4 mg/kg to dogs .
	manualset3
129261	15	405933	13	NULL	NULL	0	NULL	0.4 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats and dogs were also dosed iv for 91 days ( 3 injections/week ) with 4 ' - epidoxorubicin or doxorubicin at doses of 0.128 , 0.32 , and 0.8 mg/kg to rats and 0.064 , 0.16 , and 0.4 mg/kg to dogs .
	manualset3
129262	16	405933	13	NULL	NULL	0	NULL	dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats and dogs were also dosed iv for 91 days ( 3 injections/week ) with 4 ' - epidoxorubicin or doxorubicin at doses of 0.128 , 0.32 , and 0.8 mg/kg to rats and 0.064 , 0.16 , and 0.4 mg/kg to dogs .
	manualset3
129263	1	405934	13	NULL	NULL	0	NULL	Rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats underwent magnetic resonance angiography ( MRA ) , short-time inversion recovery ( STIR ) edema-weighed imaging , proton MR spectroscopy ( & lt ; sup & gt ; 1 & lt ; / sup & gt ; H-MRS ) , thermal infrared imaging ( IRI ) , immunoblotting and immunofluorescence analysis on both hindlimbs for 4 weeks .
	manualset3
129264	2	405934	13	NULL	NULL	0	NULL	magnetic resonance angiography ( MRA )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats underwent magnetic resonance angiography ( MRA ) , short-time inversion recovery ( STIR ) edema-weighed imaging , proton MR spectroscopy ( & lt ; sup & gt ; 1 & lt ; / sup & gt ; H-MRS ) , thermal infrared imaging ( IRI ) , immunoblotting and immunofluorescence analysis on both hindlimbs for 4 weeks .
	manualset3
129265	3	405934	13	NULL	NULL	0	NULL	short-time inversion recovery ( STIR ) edema-weighed imaging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats underwent magnetic resonance angiography ( MRA ) , short-time inversion recovery ( STIR ) edema-weighed imaging , proton MR spectroscopy ( & lt ; sup & gt ; 1 & lt ; / sup & gt ; H-MRS ) , thermal infrared imaging ( IRI ) , immunoblotting and immunofluorescence analysis on both hindlimbs for 4 weeks .
	manualset3
129266	4	405934	13	NULL	NULL	0	NULL	proton MR spectroscopy ( & lt ; sup & gt ; 1 & lt ; / sup & gt ; H-MRS )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats underwent magnetic resonance angiography ( MRA ) , short-time inversion recovery ( STIR ) edema-weighed imaging , proton MR spectroscopy ( & lt ; sup & gt ; 1 & lt ; / sup & gt ; H-MRS ) , thermal infrared imaging ( IRI ) , immunoblotting and immunofluorescence analysis on both hindlimbs for 4 weeks .
	manualset3
129267	5	405934	13	NULL	NULL	0	NULL	thermal infrared imaging ( IRI )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats underwent magnetic resonance angiography ( MRA ) , short-time inversion recovery ( STIR ) edema-weighed imaging , proton MR spectroscopy ( & lt ; sup & gt ; 1 & lt ; / sup & gt ; H-MRS ) , thermal infrared imaging ( IRI ) , immunoblotting and immunofluorescence analysis on both hindlimbs for 4 weeks .
	manualset3
129268	6	405934	13	NULL	NULL	0	NULL	immunoblotting analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats underwent magnetic resonance angiography ( MRA ) , short-time inversion recovery ( STIR ) edema-weighed imaging , proton MR spectroscopy ( & lt ; sup & gt ; 1 & lt ; / sup & gt ; H-MRS ) , thermal infrared imaging ( IRI ) , immunoblotting and immunofluorescence analysis on both hindlimbs for 4 weeks .
	manualset3
129269	7	405934	13	NULL	NULL	0	NULL	immunofluorescence analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats underwent magnetic resonance angiography ( MRA ) , short-time inversion recovery ( STIR ) edema-weighed imaging , proton MR spectroscopy ( & lt ; sup & gt ; 1 & lt ; / sup & gt ; H-MRS ) , thermal infrared imaging ( IRI ) , immunoblotting and immunofluorescence analysis on both hindlimbs for 4 weeks .
	manualset3
129270	8	405934	13	NULL	NULL	0	NULL	hindlimbs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats underwent magnetic resonance angiography ( MRA ) , short-time inversion recovery ( STIR ) edema-weighed imaging , proton MR spectroscopy ( & lt ; sup & gt ; 1 & lt ; / sup & gt ; H-MRS ) , thermal infrared imaging ( IRI ) , immunoblotting and immunofluorescence analysis on both hindlimbs for 4 weeks .
	manualset3
129271	9	405934	13	NULL	NULL	0	NULL	4 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats underwent magnetic resonance angiography ( MRA ) , short-time inversion recovery ( STIR ) edema-weighed imaging , proton MR spectroscopy ( & lt ; sup & gt ; 1 & lt ; / sup & gt ; H-MRS ) , thermal infrared imaging ( IRI ) , immunoblotting and immunofluorescence analysis on both hindlimbs for 4 weeks .
	manualset3
129272	1	405935	13	NULL	NULL	0	NULL	Rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats weighing 100 + / - 8 g were used in an in vivo kinetic study of the intestinal absorption of calcium ( CaA ) from three systems : 1 ) CaCl2 , 2 ) whole cow 's milk ( M ) , and 3 ) a staple Brazilian diet ( SBD ) .
	manualset3
129273	2	405935	13	NULL	NULL	0	NULL	100 + / - 8 g	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats weighing 100 + / - 8 g were used in an in vivo kinetic study of the intestinal absorption of calcium ( CaA ) from three systems : 1 ) CaCl2 , 2 ) whole cow 's milk ( M ) , and 3 ) a staple Brazilian diet ( SBD ) .
	manualset3
129274	3	405935	13	NULL	NULL	0	NULL	in vivo kinetic study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats weighing 100 + / - 8 g were used in an in vivo kinetic study of the intestinal absorption of calcium ( CaA ) from three systems : 1 ) CaCl2 , 2 ) whole cow 's milk ( M ) , and 3 ) a staple Brazilian diet ( SBD ) .
	manualset3
129275	4	405935	13	NULL	NULL	0	NULL	intestinal absorption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats weighing 100 + / - 8 g were used in an in vivo kinetic study of the intestinal absorption of calcium ( CaA ) from three systems : 1 ) CaCl2 , 2 ) whole cow 's milk ( M ) , and 3 ) a staple Brazilian diet ( SBD ) .
	manualset3
129276	5	405935	13	NULL	NULL	0	NULL	calcium ( CaA )	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats weighing 100 + / - 8 g were used in an in vivo kinetic study of the intestinal absorption of calcium ( CaA ) from three systems : 1 ) CaCl2 , 2 ) whole cow 's milk ( M ) , and 3 ) a staple Brazilian diet ( SBD ) .
	manualset3
129277	6	405935	13	NULL	NULL	0	NULL	three systems	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats weighing 100 + / - 8 g were used in an in vivo kinetic study of the intestinal absorption of calcium ( CaA ) from three systems : 1 ) CaCl2 , 2 ) whole cow 's milk ( M ) , and 3 ) a staple Brazilian diet ( SBD ) .
	manualset3
129278	7	405935	13	NULL	NULL	0	NULL	CaCl2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats weighing 100 + / - 8 g were used in an in vivo kinetic study of the intestinal absorption of calcium ( CaA ) from three systems : 1 ) CaCl2 , 2 ) whole cow 's milk ( M ) , and 3 ) a staple Brazilian diet ( SBD ) .
	manualset3
129279	8	405935	13	NULL	NULL	0	NULL	whole cow 's milk ( M ) 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats weighing 100 + / - 8 g were used in an in vivo kinetic study of the intestinal absorption of calcium ( CaA ) from three systems : 1 ) CaCl2 , 2 ) whole cow 's milk ( M ) , and 3 ) a staple Brazilian diet ( SBD ) .
	manualset3
129280	9	405935	13	NULL	NULL	0	NULL	staple Brazilian diet ( SBD )	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats weighing 100 + / - 8 g were used in an in vivo kinetic study of the intestinal absorption of calcium ( CaA ) from three systems : 1 ) CaCl2 , 2 ) whole cow 's milk ( M ) , and 3 ) a staple Brazilian diet ( SBD ) .
	manualset3
129281	1	405936	13	NULL	NULL	0	NULL	Rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were OVX on diestrous day 2 , treated with 30 microg estradiol benzoate or oil vehicle , sc , and then administered either oil vehicle or the type I antiprogestin , ZK98299 at 0900 h on proestrus .
	manualset3
129282	2	405936	13	NULL	NULL	0	NULL	diestrous day 2	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were OVX on diestrous day 2 , treated with 30 microg estradiol benzoate or oil vehicle , sc , and then administered either oil vehicle or the type I antiprogestin , ZK98299 at 0900 h on proestrus .
	manualset3
129283	3	405936	13	NULL	NULL	0	NULL	30 microg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were OVX on diestrous day 2 , treated with 30 microg estradiol benzoate or oil vehicle , sc , and then administered either oil vehicle or the type I antiprogestin , ZK98299 at 0900 h on proestrus .
	manualset3
129284	4	405936	13	NULL	NULL	0	NULL	estradiol benzoate	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were OVX on diestrous day 2 , treated with 30 microg estradiol benzoate or oil vehicle , sc , and then administered either oil vehicle or the type I antiprogestin , ZK98299 at 0900 h on proestrus .
	manualset3
129285	5	405936	13	NULL	NULL	0	NULL	oil vehicle	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were OVX on diestrous day 2 , treated with 30 microg estradiol benzoate or oil vehicle , sc , and then administered either oil vehicle or the type I antiprogestin , ZK98299 at 0900 h on proestrus .
	manualset3
129286	6	405936	13	NULL	NULL	0	NULL	sc	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were OVX on diestrous day 2 , treated with 30 microg estradiol benzoate or oil vehicle , sc , and then administered either oil vehicle or the type I antiprogestin , ZK98299 at 0900 h on proestrus .
	manualset3
129287	7	405936	13	NULL	NULL	0	NULL	oil vehicle 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were OVX on diestrous day 2 , treated with 30 microg estradiol benzoate or oil vehicle , sc , and then administered either oil vehicle or the type I antiprogestin , ZK98299 at 0900 h on proestrus .
	manualset3
129288	8	405936	13	NULL	NULL	NULL	NULL	type I antiprogestin	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Rats were OVX on diestrous day 2 , treated with 30 microg estradiol benzoate or oil vehicle , sc , and then administered either oil vehicle or the type I antiprogestin , ZK98299 at 0900 h on proestrus .
	manualset3
129289	9	405936	13	NULL	NULL	0	NULL	ZK98299	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were OVX on diestrous day 2 , treated with 30 microg estradiol benzoate or oil vehicle , sc , and then administered either oil vehicle or the type I antiprogestin , ZK98299 at 0900 h on proestrus .
	manualset3
129290	10	405936	13	NULL	NULL	0	NULL	0900 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were OVX on diestrous day 2 , treated with 30 microg estradiol benzoate or oil vehicle , sc , and then administered either oil vehicle or the type I antiprogestin , ZK98299 at 0900 h on proestrus .
	manualset3
129291	11	405936	13	NULL	NULL	0	NULL	proestrus	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were OVX on diestrous day 2 , treated with 30 microg estradiol benzoate or oil vehicle , sc , and then administered either oil vehicle or the type I antiprogestin , ZK98299 at 0900 h on proestrus .
	manualset3
129309	1	405937	13	NULL	NULL	0	NULL	Capillary permeability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Capillary permeability and microcirculation in the area of affected joints in infectious nonspecific polyarthritis ( according to the data of the radioisotope dilution technic ) ) .
	manualset3
129310	2	405937	13	NULL	NULL	0	NULL	microcirculation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Capillary permeability and microcirculation in the area of affected joints in infectious nonspecific polyarthritis ( according to the data of the radioisotope dilution technic ) ) .
	manualset3
129311	3	405937	13	NULL	NULL	0	NULL	area	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Capillary permeability and microcirculation in the area of affected joints in infectious nonspecific polyarthritis ( according to the data of the radioisotope dilution technic ) ) .
	manualset3
129312	4	405937	13	NULL	NULL	0	NULL	joints	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Capillary permeability and microcirculation in the area of affected joints in infectious nonspecific polyarthritis ( according to the data of the radioisotope dilution technic ) ) .
	manualset3
129313	5	405937	13	NULL	NULL	0	NULL	infectious nonspecific polyarthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Capillary permeability and microcirculation in the area of affected joints in infectious nonspecific polyarthritis ( according to the data of the radioisotope dilution technic ) ) .
	manualset3
129314	6	405937	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Capillary permeability and microcirculation in the area of affected joints in infectious nonspecific polyarthritis ( according to the data of the radioisotope dilution technic ) ) .
	manualset3
129315	7	405937	13	NULL	NULL	0	NULL	radioisotope dilution technic	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Capillary permeability and microcirculation in the area of affected joints in infectious nonspecific polyarthritis ( according to the data of the radioisotope dilution technic ) ) .
	manualset3
129316	1	405938	13	NULL	NULL	0	NULL	method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for the sequential extraction and profiling by two-dimensional gel electrophoresis ( 2-DE ) of Medicago sativa ( alfalfa ) stem cell wall proteins is described .
	manualset3
129317	2	405938	13	NULL	NULL	0	NULL	sequential extraction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for the sequential extraction and profiling by two-dimensional gel electrophoresis ( 2-DE ) of Medicago sativa ( alfalfa ) stem cell wall proteins is described .
	manualset3
129318	3	405938	13	NULL	NULL	0	NULL	profiling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for the sequential extraction and profiling by two-dimensional gel electrophoresis ( 2-DE ) of Medicago sativa ( alfalfa ) stem cell wall proteins is described .
	manualset3
129319	4	405938	13	NULL	NULL	0	NULL	 two-dimensional gel electrophoresis ( 2-DE )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for the sequential extraction and profiling by two-dimensional gel electrophoresis ( 2-DE ) of Medicago sativa ( alfalfa ) stem cell wall proteins is described .
	manualset3
129320	5	405938	13	NULL	NULL	0	NULL	Medicago sativa ( alfalfa ) stem cell wall proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A method for the sequential extraction and profiling by two-dimensional gel electrophoresis ( 2-DE ) of Medicago sativa ( alfalfa ) stem cell wall proteins is described .
	manualset3
129321	1	405939	13	NULL	NULL	0	NULL	Rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were exposed to testosterone propionate ( TP ) or vehicle from E20 to postnatal day 10 ( PN10 ) or until the time of sacrifice .
	manualset3
129322	2	405939	13	NULL	NULL	0	NULL	testosterone propionate ( TP ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were exposed to testosterone propionate ( TP ) or vehicle from E20 to postnatal day 10 ( PN10 ) or until the time of sacrifice .
	manualset3
129323	3	405939	13	NULL	NULL	0	NULL	vehicle	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were exposed to testosterone propionate ( TP ) or vehicle from E20 to postnatal day 10 ( PN10 ) or until the time of sacrifice .
	manualset3
129324	4	405939	13	NULL	NULL	0	NULL	E20	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were exposed to testosterone propionate ( TP ) or vehicle from E20 to postnatal day 10 ( PN10 ) or until the time of sacrifice .
	manualset3
129325	5	405939	13	NULL	NULL	0	NULL	postnatal day 10 ( PN10 )	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were exposed to testosterone propionate ( TP ) or vehicle from E20 to postnatal day 10 ( PN10 ) or until the time of sacrifice .
	manualset3
129326	6	405939	13	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were exposed to testosterone propionate ( TP ) or vehicle from E20 to postnatal day 10 ( PN10 ) or until the time of sacrifice .
	manualset3
129327	7	405939	13	NULL	NULL	0	NULL	sacrifice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were exposed to testosterone propionate ( TP ) or vehicle from E20 to postnatal day 10 ( PN10 ) or until the time of sacrifice .
	manualset3
129328	1	405940	13	NULL	NULL	0	NULL	Rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were given drinking water containing 2.5 g/l of DAP ad libitum and received alternate-day injections of 1 mg/kg body weight of tetragastrin in depot form after 25 weeks of oral treatment with MNNG .
	manualset3
129329	2	405940	13	NULL	NULL	0	NULL	drinking water	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were given drinking water containing 2.5 g/l of DAP ad libitum and received alternate-day injections of 1 mg/kg body weight of tetragastrin in depot form after 25 weeks of oral treatment with MNNG .
	manualset3
129330	3	405940	13	NULL	NULL	0	NULL	2.5 g/l 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were given drinking water containing 2.5 g/l of DAP ad libitum and received alternate-day injections of 1 mg/kg body weight of tetragastrin in depot form after 25 weeks of oral treatment with MNNG .
	manualset3
129331	4	405940	13	NULL	NULL	0	NULL	DAP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were given drinking water containing 2.5 g/l of DAP ad libitum and received alternate-day injections of 1 mg/kg body weight of tetragastrin in depot form after 25 weeks of oral treatment with MNNG .
	manualset3
129332	5	405940	13	NULL	NULL	NULL	NULL	ad libitum	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Rats were given drinking water containing 2.5 g/l of DAP ad libitum and received alternate-day injections of 1 mg/kg body weight of tetragastrin in depot form after 25 weeks of oral treatment with MNNG .
	manualset3
129333	6	405940	13	NULL	NULL	0	NULL	alternate-day injections	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were given drinking water containing 2.5 g/l of DAP ad libitum and received alternate-day injections of 1 mg/kg body weight of tetragastrin in depot form after 25 weeks of oral treatment with MNNG .
	manualset3
129334	7	405940	13	NULL	NULL	0	NULL	1 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were given drinking water containing 2.5 g/l of DAP ad libitum and received alternate-day injections of 1 mg/kg body weight of tetragastrin in depot form after 25 weeks of oral treatment with MNNG .
	manualset3
129335	8	405940	13	NULL	NULL	0	NULL	body weight 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were given drinking water containing 2.5 g/l of DAP ad libitum and received alternate-day injections of 1 mg/kg body weight of tetragastrin in depot form after 25 weeks of oral treatment with MNNG .
	manualset3
129336	9	405940	13	NULL	NULL	0	NULL	tetragastrin	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were given drinking water containing 2.5 g/l of DAP ad libitum and received alternate-day injections of 1 mg/kg body weight of tetragastrin in depot form after 25 weeks of oral treatment with MNNG .
	manualset3
129337	10	405940	13	NULL	NULL	0	NULL	25 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were given drinking water containing 2.5 g/l of DAP ad libitum and received alternate-day injections of 1 mg/kg body weight of tetragastrin in depot form after 25 weeks of oral treatment with MNNG .
	manualset3
129338	11	405940	13	NULL	NULL	0	NULL	oral treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were given drinking water containing 2.5 g/l of DAP ad libitum and received alternate-day injections of 1 mg/kg body weight of tetragastrin in depot form after 25 weeks of oral treatment with MNNG .
	manualset3
129339	12	405940	13	NULL	NULL	0	NULL	MNNG	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were given drinking water containing 2.5 g/l of DAP ad libitum and received alternate-day injections of 1 mg/kg body weight of tetragastrin in depot form after 25 weeks of oral treatment with MNNG .
	manualset3
129340	1	405941	13	NULL	NULL	0	NULL	Rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were injected with a borderline toxic dose of glycerol and 24 hours later proximal tubular segments ( PTS ) were isolated for study .
	manualset3
129341	2	405941	13	NULL	NULL	0	NULL	toxic dose	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were injected with a borderline toxic dose of glycerol and 24 hours later proximal tubular segments ( PTS ) were isolated for study .
	manualset3
129342	3	405941	13	NULL	NULL	0	NULL	glycerol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were injected with a borderline toxic dose of glycerol and 24 hours later proximal tubular segments ( PTS ) were isolated for study .
	manualset3
129343	4	405941	13	NULL	NULL	0	NULL	24 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were injected with a borderline toxic dose of glycerol and 24 hours later proximal tubular segments ( PTS ) were isolated for study .
	manualset3
129344	5	405941	13	NULL	NULL	0	NULL	proximal tubular segments ( PTS )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were injected with a borderline toxic dose of glycerol and 24 hours later proximal tubular segments ( PTS ) were isolated for study .
	manualset3
129345	6	405941	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were injected with a borderline toxic dose of glycerol and 24 hours later proximal tubular segments ( PTS ) were isolated for study .
	manualset3
129346	1	405942	13	NULL	NULL	0	NULL	Rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were killed either immediately or 2 to 4 weeks after surgery .
	manualset3
129347	2	405942	13	NULL	NULL	0	NULL	 2 to 4 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were killed either immediately or 2 to 4 weeks after surgery .
	manualset3
129348	3	405942	13	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were killed either immediately or 2 to 4 weeks after surgery .
	manualset3
129349	1	405943	13	NULL	NULL	0	NULL	Rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats with lesions of the ventral subiculum ( vSUB ) or ventral hippocampus ( vHIPPO ) did not show changes in basal corticosterone ( CORT ) secretion at either circadian peak or nadir time points when compared to sham-lesion rats ( SHAM ) or unoperated controls .
	manualset3
129350	2	405943	13	NULL	NULL	0	NULL	lesions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats with lesions of the ventral subiculum ( vSUB ) or ventral hippocampus ( vHIPPO ) did not show changes in basal corticosterone ( CORT ) secretion at either circadian peak or nadir time points when compared to sham-lesion rats ( SHAM ) or unoperated controls .
	manualset3
129351	3	405943	13	NULL	NULL	0	NULL	 ventral subiculum ( vSUB ) 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats with lesions of the ventral subiculum ( vSUB ) or ventral hippocampus ( vHIPPO ) did not show changes in basal corticosterone ( CORT ) secretion at either circadian peak or nadir time points when compared to sham-lesion rats ( SHAM ) or unoperated controls .
	manualset3
129352	4	405943	13	NULL	NULL	0	NULL	ventral hippocampus ( vHIPPO ) 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats with lesions of the ventral subiculum ( vSUB ) or ventral hippocampus ( vHIPPO ) did not show changes in basal corticosterone ( CORT ) secretion at either circadian peak or nadir time points when compared to sham-lesion rats ( SHAM ) or unoperated controls .
	manualset3
129353	5	405943	13	NULL	NULL	0	NULL	changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats with lesions of the ventral subiculum ( vSUB ) or ventral hippocampus ( vHIPPO ) did not show changes in basal corticosterone ( CORT ) secretion at either circadian peak or nadir time points when compared to sham-lesion rats ( SHAM ) or unoperated controls .
	manualset3
129354	6	405943	13	NULL	NULL	0	NULL	basal corticosterone ( CORT ) secretion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats with lesions of the ventral subiculum ( vSUB ) or ventral hippocampus ( vHIPPO ) did not show changes in basal corticosterone ( CORT ) secretion at either circadian peak or nadir time points when compared to sham-lesion rats ( SHAM ) or unoperated controls .
	manualset3
129355	7	405943	13	NULL	NULL	0	NULL	circadian peak 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats with lesions of the ventral subiculum ( vSUB ) or ventral hippocampus ( vHIPPO ) did not show changes in basal corticosterone ( CORT ) secretion at either circadian peak or nadir time points when compared to sham-lesion rats ( SHAM ) or unoperated controls .
	manualset3
129356	8	405943	13	NULL	NULL	0	NULL	nadir time points	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats with lesions of the ventral subiculum ( vSUB ) or ventral hippocampus ( vHIPPO ) did not show changes in basal corticosterone ( CORT ) secretion at either circadian peak or nadir time points when compared to sham-lesion rats ( SHAM ) or unoperated controls .
	manualset3
129357	9	405943	13	NULL	NULL	0	NULL	sham-lesion rats ( SHAM )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats with lesions of the ventral subiculum ( vSUB ) or ventral hippocampus ( vHIPPO ) did not show changes in basal corticosterone ( CORT ) secretion at either circadian peak or nadir time points when compared to sham-lesion rats ( SHAM ) or unoperated controls .
	manualset3
129358	10	405943	13	NULL	NULL	0	NULL	controls	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats with lesions of the ventral subiculum ( vSUB ) or ventral hippocampus ( vHIPPO ) did not show changes in basal corticosterone ( CORT ) secretion at either circadian peak or nadir time points when compared to sham-lesion rats ( SHAM ) or unoperated controls .
	manualset3
129359	1	405944	13	NULL	NULL	0	NULL	Re-amputation rate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Re-amputation rate to a more proximal level was significantly higher in BKA compared with GSA .
	manualset3
129360	2	405944	13	NULL	NULL	0	NULL	proximal level	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Re-amputation rate to a more proximal level was significantly higher in BKA compared with GSA .
	manualset3
129361	3	405944	13	NULL	NULL	0	NULL	BKA 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Re-amputation rate to a more proximal level was significantly higher in BKA compared with GSA .
	manualset3
129362	4	405944	13	NULL	NULL	0	NULL	GSA	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Re-amputation rate to a more proximal level was significantly higher in BKA compared with GSA .
	manualset3
129363	1	405945	13	NULL	NULL	0	NULL	method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A method is described in which the interaction between thrombin and platelet proteins can be studied directly .
	manualset3
129364	2	405945	13	NULL	NULL	0	NULL	interaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A method is described in which the interaction between thrombin and platelet proteins can be studied directly .
	manualset3
129365	3	405945	13	NULL	NULL	0	NULL	thrombin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A method is described in which the interaction between thrombin and platelet proteins can be studied directly .
	manualset3
129366	4	405945	13	NULL	NULL	0	NULL	platelet proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A method is described in which the interaction between thrombin and platelet proteins can be studied directly .
	manualset3
129367	1	405946	13	NULL	NULL	0	NULL	Re-click deficits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Re-click deficits correlated with degree of leftward neglect , mainly due to both being severe in intraparietal cases .
	manualset3
129368	2	405946	13	NULL	NULL	0	NULL	degree	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Re-click deficits correlated with degree of leftward neglect , mainly due to both being severe in intraparietal cases .
	manualset3
129369	3	405946	13	NULL	NULL	0	NULL	leftward neglect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Re-click deficits correlated with degree of leftward neglect , mainly due to both being severe in intraparietal cases .
	manualset3
129370	4	405946	13	NULL	NULL	0	NULL	intraparietal cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Re-click deficits correlated with degree of leftward neglect , mainly due to both being severe in intraparietal cases .
	manualset3
129371	1	405947	13	NULL	NULL	0	NULL	Re-treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Re-treatment of pulmonary tuberculosis with rifampin and ethambutol .
	manualset3
129372	2	405947	13	NULL	NULL	0	NULL	pulmonary tuberculosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Re-treatment of pulmonary tuberculosis with rifampin and ethambutol .
	manualset3
129373	3	405947	13	NULL	NULL	0	NULL	rifampin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Re-treatment of pulmonary tuberculosis with rifampin and ethambutol .
	manualset3
129374	4	405947	13	NULL	NULL	0	NULL	ethambutol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Re-treatment of pulmonary tuberculosis with rifampin and ethambutol .
	manualset3
129375	1	405948	13	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Re : The relationship between childhood behavior disorders and unintentional injury events .
	manualset3
129376	2	405948	13	NULL	NULL	0	NULL	childhood behavior disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Re : The relationship between childhood behavior disorders and unintentional injury events .
	manualset3
129377	3	405948	13	NULL	NULL	0	NULL	unintentional injury events	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Re : The relationship between childhood behavior disorders and unintentional injury events .
	manualset3
129378	1	405949	13	NULL	NULL	0	NULL	Reaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reaction between ( PPh4 ) ( closo-4-CB8H9 ) and ( Ru3 ( CO ) 12 ) in refluxing toluene affords the unprecedented hexaruthenium metallacarborane salt ( PPh4 ) ( 2 , 3 , 7 - { Ru ( CO ) 3 } -2 , 6 , 11 - { Ru ( CO ) 3 } -7 , 11 , 12 - { Ru ( CO ) 3 } -3 , 6 , 12 - ( micro-H ) 3-2 , 2 , 7 , 7 , 11 , 11 - ( CO ) 6-closo-2 , 7 , 11 , 1 - Ru3CB8H6 ) ( 1a ) , which contains a planar Ru6 ` raft ' supported by a { CB8 } monocarborane cluster .
	manualset3
129379	2	405949	13	NULL	NULL	0	NULL	( PPh4 ) ( closo-4-CB8H9 ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Reaction between ( PPh4 ) ( closo-4-CB8H9 ) and ( Ru3 ( CO ) 12 ) in refluxing toluene affords the unprecedented hexaruthenium metallacarborane salt ( PPh4 ) ( 2 , 3 , 7 - { Ru ( CO ) 3 } -2 , 6 , 11 - { Ru ( CO ) 3 } -7 , 11 , 12 - { Ru ( CO ) 3 } -3 , 6 , 12 - ( micro-H ) 3-2 , 2 , 7 , 7 , 11 , 11 - ( CO ) 6-closo-2 , 7 , 11 , 1 - Ru3CB8H6 ) ( 1a ) , which contains a planar Ru6 ` raft ' supported by a { CB8 } monocarborane cluster .
	manualset3
129380	3	405949	13	NULL	NULL	0	NULL	( Ru3 ( CO ) 12 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Reaction between ( PPh4 ) ( closo-4-CB8H9 ) and ( Ru3 ( CO ) 12 ) in refluxing toluene affords the unprecedented hexaruthenium metallacarborane salt ( PPh4 ) ( 2 , 3 , 7 - { Ru ( CO ) 3 } -2 , 6 , 11 - { Ru ( CO ) 3 } -7 , 11 , 12 - { Ru ( CO ) 3 } -3 , 6 , 12 - ( micro-H ) 3-2 , 2 , 7 , 7 , 11 , 11 - ( CO ) 6-closo-2 , 7 , 11 , 1 - Ru3CB8H6 ) ( 1a ) , which contains a planar Ru6 ` raft ' supported by a { CB8 } monocarborane cluster .
	manualset3
129381	4	405949	13	NULL	NULL	0	NULL	toluene 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Reaction between ( PPh4 ) ( closo-4-CB8H9 ) and ( Ru3 ( CO ) 12 ) in refluxing toluene affords the unprecedented hexaruthenium metallacarborane salt ( PPh4 ) ( 2 , 3 , 7 - { Ru ( CO ) 3 } -2 , 6 , 11 - { Ru ( CO ) 3 } -7 , 11 , 12 - { Ru ( CO ) 3 } -3 , 6 , 12 - ( micro-H ) 3-2 , 2 , 7 , 7 , 11 , 11 - ( CO ) 6-closo-2 , 7 , 11 , 1 - Ru3CB8H6 ) ( 1a ) , which contains a planar Ru6 ` raft ' supported by a { CB8 } monocarborane cluster .
	manualset3
129382	5	405949	13	NULL	NULL	0	NULL	hexaruthenium metallacarborane salt 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Reaction between ( PPh4 ) ( closo-4-CB8H9 ) and ( Ru3 ( CO ) 12 ) in refluxing toluene affords the unprecedented hexaruthenium metallacarborane salt ( PPh4 ) ( 2 , 3 , 7 - { Ru ( CO ) 3 } -2 , 6 , 11 - { Ru ( CO ) 3 } -7 , 11 , 12 - { Ru ( CO ) 3 } -3 , 6 , 12 - ( micro-H ) 3-2 , 2 , 7 , 7 , 11 , 11 - ( CO ) 6-closo-2 , 7 , 11 , 1 - Ru3CB8H6 ) ( 1a ) , which contains a planar Ru6 ` raft ' supported by a { CB8 } monocarborane cluster .
	manualset3
129383	6	405949	13	NULL	NULL	0	NULL	( PPh4 ) ( 2 , 3 , 7 - { Ru ( CO ) 3 } -2 , 6 , 11 - { Ru ( CO ) 3 } -7 , 11 , 12 - { Ru ( CO ) 3 } -3 , 6 , 12 - ( micro-H ) 3-2 , 2 , 7 , 7 , 11 , 11 - ( CO ) 6-closo-2 , 7 , 11 , 1 - Ru3CB8H6 ) ( 1a ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Reaction between ( PPh4 ) ( closo-4-CB8H9 ) and ( Ru3 ( CO ) 12 ) in refluxing toluene affords the unprecedented hexaruthenium metallacarborane salt ( PPh4 ) ( 2 , 3 , 7 - { Ru ( CO ) 3 } -2 , 6 , 11 - { Ru ( CO ) 3 } -7 , 11 , 12 - { Ru ( CO ) 3 } -3 , 6 , 12 - ( micro-H ) 3-2 , 2 , 7 , 7 , 11 , 11 - ( CO ) 6-closo-2 , 7 , 11 , 1 - Ru3CB8H6 ) ( 1a ) , which contains a planar Ru6 ` raft ' supported by a { CB8 } monocarborane cluster .
	manualset3
129384	7	405949	13	NULL	NULL	0	NULL	planar Ru6 ` raft ' 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Reaction between ( PPh4 ) ( closo-4-CB8H9 ) and ( Ru3 ( CO ) 12 ) in refluxing toluene affords the unprecedented hexaruthenium metallacarborane salt ( PPh4 ) ( 2 , 3 , 7 - { Ru ( CO ) 3 } -2 , 6 , 11 - { Ru ( CO ) 3 } -7 , 11 , 12 - { Ru ( CO ) 3 } -3 , 6 , 12 - ( micro-H ) 3-2 , 2 , 7 , 7 , 11 , 11 - ( CO ) 6-closo-2 , 7 , 11 , 1 - Ru3CB8H6 ) ( 1a ) , which contains a planar Ru6 ` raft ' supported by a { CB8 } monocarborane cluster .
	manualset3
129385	8	405949	13	NULL	NULL	0	NULL	{ CB8 } monocarborane cluster	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Reaction between ( PPh4 ) ( closo-4-CB8H9 ) and ( Ru3 ( CO ) 12 ) in refluxing toluene affords the unprecedented hexaruthenium metallacarborane salt ( PPh4 ) ( 2 , 3 , 7 - { Ru ( CO ) 3 } -2 , 6 , 11 - { Ru ( CO ) 3 } -7 , 11 , 12 - { Ru ( CO ) 3 } -3 , 6 , 12 - ( micro-H ) 3-2 , 2 , 7 , 7 , 11 , 11 - ( CO ) 6-closo-2 , 7 , 11 , 1 - Ru3CB8H6 ) ( 1a ) , which contains a planar Ru6 ` raft ' supported by a { CB8 } monocarborane cluster .
	manualset3
129386	1	405950	13	NULL	NULL	0	NULL	Reaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reaction of isophthalic acid ( isophH ( 2 ) ) with manganese ( II ) acetate results in the formation of ( Mn ( isoph ) ) .2 H ( 2 ) O ( 4 ) .
	manualset3
129387	2	405950	13	NULL	NULL	0	NULL	isophthalic acid ( isophH ( 2 ) )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Reaction of isophthalic acid ( isophH ( 2 ) ) with manganese ( II ) acetate results in the formation of ( Mn ( isoph ) ) .2 H ( 2 ) O ( 4 ) .
	manualset3
129388	3	405950	13	NULL	NULL	0	NULL	manganese ( II ) acetate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Reaction of isophthalic acid ( isophH ( 2 ) ) with manganese ( II ) acetate results in the formation of ( Mn ( isoph ) ) .2 H ( 2 ) O ( 4 ) .
	manualset3
129390	5	405950	13	NULL	NULL	0	NULL	formation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reaction of isophthalic acid ( isophH ( 2 ) ) with manganese ( II ) acetate results in the formation of ( Mn ( isoph ) ) .2 H ( 2 ) O ( 4 ) .
	manualset3
129391	6	405950	13	NULL	NULL	0	NULL	( Mn ( isoph ) ) .2 H ( 2 ) O ( 4 ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Reaction of isophthalic acid ( isophH ( 2 ) ) with manganese ( II ) acetate results in the formation of ( Mn ( isoph ) ) .2 H ( 2 ) O ( 4 ) .
	manualset3
129392	1	405951	13	NULL	NULL	0	NULL	Reaction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reaction of thallium ( III ) salts with homoallylic alcohols : ring contraction vs. dimethoxylation .
	manualset3
129393	2	405951	13	NULL	NULL	0	NULL	thallium ( III ) salts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Reaction of thallium ( III ) salts with homoallylic alcohols : ring contraction vs. dimethoxylation .
	manualset3
129394	3	405951	13	NULL	NULL	0	NULL	homoallylic alcohols	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Reaction of thallium ( III ) salts with homoallylic alcohols : ring contraction vs. dimethoxylation .
	manualset3
129395	4	405951	13	NULL	NULL	0	NULL	ring contraction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reaction of thallium ( III ) salts with homoallylic alcohols : ring contraction vs. dimethoxylation .
	manualset3
129396	5	405951	13	NULL	NULL	0	NULL	dimethoxylation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reaction of thallium ( III ) salts with homoallylic alcohols : ring contraction vs. dimethoxylation .
	manualset3
129397	1	405952	13	NULL	NULL	0	NULL	method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A method of determining electrical potential gradient across mitochondrial membrane in perfused rat hearts .
	manualset3
129398	2	405952	13	NULL	NULL	0	NULL	electrical potential gradient 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A method of determining electrical potential gradient across mitochondrial membrane in perfused rat hearts .
	manualset3
129399	3	405952	13	NULL	NULL	0	NULL	mitochondrial membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A method of determining electrical potential gradient across mitochondrial membrane in perfused rat hearts .
	manualset3
129400	4	405952	13	NULL	NULL	0	NULL	rat hearts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A method of determining electrical potential gradient across mitochondrial membrane in perfused rat hearts .
	manualset3
129401	1	405953	13	NULL	NULL	0	NULL	Reactions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reactions of alkenes with OH , NO3 and O3 .
	manualset3
129402	2	405953	13	NULL	NULL	0	NULL	alkenes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Reactions of alkenes with OH , NO3 and O3 .
	manualset3
129403	3	405953	13	NULL	NULL	0	NULL	OH 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Reactions of alkenes with OH , NO3 and O3 .
	manualset3
129404	4	405953	13	NULL	NULL	0	NULL	NO3	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Reactions of alkenes with OH , NO3 and O3 .
	manualset3
129405	5	405953	13	NULL	NULL	0	NULL	O3	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Reactions of alkenes with OH , NO3 and O3 .
	manualset3
129406	1	405954	13	NULL	NULL	0	NULL	Reactive changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reactive changes in different topographic zones being a morphological manifestation of the immune response to the presence of tumor depend on the type and localization of the tumor .
	manualset3
129407	2	405954	13	NULL	NULL	0	NULL	topographic zones	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reactive changes in different topographic zones being a morphological manifestation of the immune response to the presence of tumor depend on the type and localization of the tumor .
	manualset3
129408	3	405954	13	NULL	NULL	0	NULL	morphological manifestation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reactive changes in different topographic zones being a morphological manifestation of the immune response to the presence of tumor depend on the type and localization of the tumor .
	manualset3
129409	4	405954	13	NULL	NULL	0	NULL	immune response 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reactive changes in different topographic zones being a morphological manifestation of the immune response to the presence of tumor depend on the type and localization of the tumor .
	manualset3
129410	5	405954	13	NULL	NULL	0	NULL	presence of tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reactive changes in different topographic zones being a morphological manifestation of the immune response to the presence of tumor depend on the type and localization of the tumor .
	manualset3
129411	6	405954	13	NULL	NULL	0	NULL	type	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reactive changes in different topographic zones being a morphological manifestation of the immune response to the presence of tumor depend on the type and localization of the tumor .
	manualset3
129412	7	405954	13	NULL	NULL	0	NULL	localization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reactive changes in different topographic zones being a morphological manifestation of the immune response to the presence of tumor depend on the type and localization of the tumor .
	manualset3
129413	8	405954	13	NULL	NULL	0	NULL	tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reactive changes in different topographic zones being a morphological manifestation of the immune response to the presence of tumor depend on the type and localization of the tumor .
	manualset3
129414	1	405955	13	NULL	NULL	0	NULL	Reactive oxygen species ( ROS ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Reactive oxygen species ( ROS ) have been implicated in the pathogenesis of toxic , ischemic and immunologically-mediated renal injury .
	manualset3
129415	2	405955	13	NULL	NULL	0	NULL	pathogenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reactive oxygen species ( ROS ) have been implicated in the pathogenesis of toxic , ischemic and immunologically-mediated renal injury .
	manualset3
129416	3	405955	13	NULL	NULL	0	NULL	toxic renal injury 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reactive oxygen species ( ROS ) have been implicated in the pathogenesis of toxic , ischemic and immunologically-mediated renal injury .
	manualset3
129417	4	405955	13	NULL	NULL	0	NULL	ischemic renal injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reactive oxygen species ( ROS ) have been implicated in the pathogenesis of toxic , ischemic and immunologically-mediated renal injury .
	manualset3
129418	5	405955	13	NULL	NULL	0	NULL	immunologically-mediated renal injury 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reactive oxygen species ( ROS ) have been implicated in the pathogenesis of toxic , ischemic and immunologically-mediated renal injury .
	manualset3
129419	1	405956	13	NULL	NULL	0	NULL	Real-time 3D echocardiography ( RT3DE )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Real-time 3D echocardiography ( RT3DE ) allows rapid and accurate semi-automated extraction of LV endocardial surfaces .
	manualset3
129420	2	405956	13	NULL	NULL	0	NULL	extraction	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Real-time 3D echocardiography ( RT3DE ) allows rapid and accurate semi-automated extraction of LV endocardial surfaces .
	manualset3
129421	3	405956	13	NULL	NULL	0	NULL	LV endocardial surfaces	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Real-time 3D echocardiography ( RT3DE ) allows rapid and accurate semi-automated extraction of LV endocardial surfaces .
	manualset3
129422	1	405957	13	NULL	NULL	0	NULL	Real-time RT-PCR analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Real-time RT-PCR analyses showed that S1P receptors S1P1 , S1P2 , and S1P3 were most abundantly expressed in the renal medulla .
	manualset3
129423	2	405957	13	NULL	NULL	0	NULL	S1P receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Real-time RT-PCR analyses showed that S1P receptors S1P1 , S1P2 , and S1P3 were most abundantly expressed in the renal medulla .
	manualset3
129424	3	405957	13	NULL	NULL	0	NULL	S1P1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Real-time RT-PCR analyses showed that S1P receptors S1P1 , S1P2 , and S1P3 were most abundantly expressed in the renal medulla .
	manualset3
129425	4	405957	13	NULL	NULL	0	NULL	S1P2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Real-time RT-PCR analyses showed that S1P receptors S1P1 , S1P2 , and S1P3 were most abundantly expressed in the renal medulla .
	manualset3
129426	5	405957	13	NULL	NULL	0	NULL	S1P3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Real-time RT-PCR analyses showed that S1P receptors S1P1 , S1P2 , and S1P3 were most abundantly expressed in the renal medulla .
	manualset3
129427	6	405957	13	NULL	NULL	0	NULL	renal medulla 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Real-time RT-PCR analyses showed that S1P receptors S1P1 , S1P2 , and S1P3 were most abundantly expressed in the renal medulla .
	manualset3
129428	1	405958	13	NULL	NULL	NULL	NULL	Real-time two-dimensional phased array sector scanner	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Real-time two-dimensional phased array sector scanner demonstrated 2 cugdel-shaped lesions in the region of the left ventricular outflow tract through the aortic root , pendulating upward and downward floating along the blood stream .
	manualset3
129429	2	405958	13	NULL	NULL	0	NULL	2 cugdel-shaped lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Real-time two-dimensional phased array sector scanner demonstrated 2 cugdel-shaped lesions in the region of the left ventricular outflow tract through the aortic root , pendulating upward and downward floating along the blood stream .
	manualset3
129430	3	405958	13	NULL	NULL	0	NULL	region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Real-time two-dimensional phased array sector scanner demonstrated 2 cugdel-shaped lesions in the region of the left ventricular outflow tract through the aortic root , pendulating upward and downward floating along the blood stream .
	manualset3
129431	4	405958	13	NULL	NULL	0	NULL	left ventricular outflow tract 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Real-time two-dimensional phased array sector scanner demonstrated 2 cugdel-shaped lesions in the region of the left ventricular outflow tract through the aortic root , pendulating upward and downward floating along the blood stream .
	manualset3
129432	5	405958	13	NULL	NULL	0	NULL	aortic root	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Real-time two-dimensional phased array sector scanner demonstrated 2 cugdel-shaped lesions in the region of the left ventricular outflow tract through the aortic root , pendulating upward and downward floating along the blood stream .
	manualset3
129433	6	405958	13	NULL	NULL	NULL	NULL	blood stream	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Real-time two-dimensional phased array sector scanner demonstrated 2 cugdel-shaped lesions in the region of the left ventricular outflow tract through the aortic root , pendulating upward and downward floating along the blood stream .
	manualset3
129434	1	405959	13	NULL	NULL	0	NULL	Reasoning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reasoning that mRNA levels of these FSH-regulating pituitary peptides might be modulated at times of increased FSH gene expression , two in vivo models were chosen for further investigation .
	manualset3
129435	2	405959	13	NULL	NULL	0	NULL	mRNA levels 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Reasoning that mRNA levels of these FSH-regulating pituitary peptides might be modulated at times of increased FSH gene expression , two in vivo models were chosen for further investigation .
	manualset3
129436	3	405959	13	NULL	NULL	0	NULL	FSH-regulating pituitary peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Reasoning that mRNA levels of these FSH-regulating pituitary peptides might be modulated at times of increased FSH gene expression , two in vivo models were chosen for further investigation .
	manualset3
129437	4	405959	13	NULL	NULL	0	NULL	FSH gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reasoning that mRNA levels of these FSH-regulating pituitary peptides might be modulated at times of increased FSH gene expression , two in vivo models were chosen for further investigation .
	manualset3
129438	5	405959	13	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Reasoning that mRNA levels of these FSH-regulating pituitary peptides might be modulated at times of increased FSH gene expression , two in vivo models were chosen for further investigation .
	manualset3
129439	6	405959	13	NULL	NULL	0	NULL	in vivo models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Reasoning that mRNA levels of these FSH-regulating pituitary peptides might be modulated at times of increased FSH gene expression , two in vivo models were chosen for further investigation .
	manualset3
129440	7	405959	13	NULL	NULL	0	NULL	investigation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reasoning that mRNA levels of these FSH-regulating pituitary peptides might be modulated at times of increased FSH gene expression , two in vivo models were chosen for further investigation .
	manualset3
129441	1	405960	13	NULL	NULL	0	NULL	Reasons	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reasons for drainage failure were abscesses caused by internal fistulas ( 8 patients ) , pancreas involvement of the abscesses ( 5 patients ) , infected clots impossible to drain ( 3 patients ) , multiple abscesses ( 3 patients ) and persistent abscess formation despite drainage ( 2 patients ) .
	manualset3
129442	2	405960	13	NULL	NULL	0	NULL	drainage failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reasons for drainage failure were abscesses caused by internal fistulas ( 8 patients ) , pancreas involvement of the abscesses ( 5 patients ) , infected clots impossible to drain ( 3 patients ) , multiple abscesses ( 3 patients ) and persistent abscess formation despite drainage ( 2 patients ) .
	manualset3
129443	3	405960	13	NULL	NULL	0	NULL	abscesses 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reasons for drainage failure were abscesses caused by internal fistulas ( 8 patients ) , pancreas involvement of the abscesses ( 5 patients ) , infected clots impossible to drain ( 3 patients ) , multiple abscesses ( 3 patients ) and persistent abscess formation despite drainage ( 2 patients ) .
	manualset3
129444	4	405960	13	NULL	NULL	0	NULL	internal fistulas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reasons for drainage failure were abscesses caused by internal fistulas ( 8 patients ) , pancreas involvement of the abscesses ( 5 patients ) , infected clots impossible to drain ( 3 patients ) , multiple abscesses ( 3 patients ) and persistent abscess formation despite drainage ( 2 patients ) .
	manualset3
129445	5	405960	13	NULL	NULL	0	NULL	8 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Reasons for drainage failure were abscesses caused by internal fistulas ( 8 patients ) , pancreas involvement of the abscesses ( 5 patients ) , infected clots impossible to drain ( 3 patients ) , multiple abscesses ( 3 patients ) and persistent abscess formation despite drainage ( 2 patients ) .
	manualset3
129446	6	405960	13	NULL	NULL	0	NULL	pancreas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Reasons for drainage failure were abscesses caused by internal fistulas ( 8 patients ) , pancreas involvement of the abscesses ( 5 patients ) , infected clots impossible to drain ( 3 patients ) , multiple abscesses ( 3 patients ) and persistent abscess formation despite drainage ( 2 patients ) .
	manualset3
129447	7	405960	13	NULL	NULL	0	NULL	involvement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reasons for drainage failure were abscesses caused by internal fistulas ( 8 patients ) , pancreas involvement of the abscesses ( 5 patients ) , infected clots impossible to drain ( 3 patients ) , multiple abscesses ( 3 patients ) and persistent abscess formation despite drainage ( 2 patients ) .
	manualset3
129448	8	405960	13	NULL	NULL	0	NULL	abscesses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reasons for drainage failure were abscesses caused by internal fistulas ( 8 patients ) , pancreas involvement of the abscesses ( 5 patients ) , infected clots impossible to drain ( 3 patients ) , multiple abscesses ( 3 patients ) and persistent abscess formation despite drainage ( 2 patients ) .
	manualset3
129449	9	405960	13	NULL	NULL	0	NULL	5 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Reasons for drainage failure were abscesses caused by internal fistulas ( 8 patients ) , pancreas involvement of the abscesses ( 5 patients ) , infected clots impossible to drain ( 3 patients ) , multiple abscesses ( 3 patients ) and persistent abscess formation despite drainage ( 2 patients ) .
	manualset3
129450	10	405960	13	NULL	NULL	0	NULL	clots 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reasons for drainage failure were abscesses caused by internal fistulas ( 8 patients ) , pancreas involvement of the abscesses ( 5 patients ) , infected clots impossible to drain ( 3 patients ) , multiple abscesses ( 3 patients ) and persistent abscess formation despite drainage ( 2 patients ) .
	manualset3
129451	11	405960	13	NULL	NULL	0	NULL	3 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Reasons for drainage failure were abscesses caused by internal fistulas ( 8 patients ) , pancreas involvement of the abscesses ( 5 patients ) , infected clots impossible to drain ( 3 patients ) , multiple abscesses ( 3 patients ) and persistent abscess formation despite drainage ( 2 patients ) .
	manualset3
129452	12	405960	13	NULL	NULL	0	NULL	multiple abscesses 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reasons for drainage failure were abscesses caused by internal fistulas ( 8 patients ) , pancreas involvement of the abscesses ( 5 patients ) , infected clots impossible to drain ( 3 patients ) , multiple abscesses ( 3 patients ) and persistent abscess formation despite drainage ( 2 patients ) .
	manualset3
129453	13	405960	13	NULL	NULL	0	NULL	3 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Reasons for drainage failure were abscesses caused by internal fistulas ( 8 patients ) , pancreas involvement of the abscesses ( 5 patients ) , infected clots impossible to drain ( 3 patients ) , multiple abscesses ( 3 patients ) and persistent abscess formation despite drainage ( 2 patients ) .
	manualset3
129454	14	405960	13	NULL	NULL	0	NULL	abscess formation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reasons for drainage failure were abscesses caused by internal fistulas ( 8 patients ) , pancreas involvement of the abscesses ( 5 patients ) , infected clots impossible to drain ( 3 patients ) , multiple abscesses ( 3 patients ) and persistent abscess formation despite drainage ( 2 patients ) .
	manualset3
129455	15	405960	13	NULL	NULL	0	NULL	drainage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reasons for drainage failure were abscesses caused by internal fistulas ( 8 patients ) , pancreas involvement of the abscesses ( 5 patients ) , infected clots impossible to drain ( 3 patients ) , multiple abscesses ( 3 patients ) and persistent abscess formation despite drainage ( 2 patients ) .
	manualset3
129456	16	405960	13	NULL	NULL	0	NULL	2 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Reasons for drainage failure were abscesses caused by internal fistulas ( 8 patients ) , pancreas involvement of the abscesses ( 5 patients ) , infected clots impossible to drain ( 3 patients ) , multiple abscesses ( 3 patients ) and persistent abscess formation despite drainage ( 2 patients ) .
	manualset3
129457	1	405961	13	NULL	NULL	0	NULL	method	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A method that may be applied for this purpose is the Danish Budget Method which estimates the maximum amount of the additive that may be added to the food based on the functional properties of the additive , and on the categories of the food in which the additive will be used .
	manualset3
129458	2	405961	13	NULL	NULL	0	NULL	purpose	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A method that may be applied for this purpose is the Danish Budget Method which estimates the maximum amount of the additive that may be added to the food based on the functional properties of the additive , and on the categories of the food in which the additive will be used .
	manualset3
129459	3	405961	13	NULL	NULL	0	NULL	 Danish Budget Method	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A method that may be applied for this purpose is the Danish Budget Method which estimates the maximum amount of the additive that may be added to the food based on the functional properties of the additive , and on the categories of the food in which the additive will be used .
	manualset3
129460	4	405961	13	NULL	NULL	0	NULL	maximum amount	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A method that may be applied for this purpose is the Danish Budget Method which estimates the maximum amount of the additive that may be added to the food based on the functional properties of the additive , and on the categories of the food in which the additive will be used .
	manualset3
129461	5	405961	13	NULL	NULL	0	NULL	additive	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A method that may be applied for this purpose is the Danish Budget Method which estimates the maximum amount of the additive that may be added to the food based on the functional properties of the additive , and on the categories of the food in which the additive will be used .
	manualset3
129462	6	405961	13	NULL	NULL	0	NULL	food	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A method that may be applied for this purpose is the Danish Budget Method which estimates the maximum amount of the additive that may be added to the food based on the functional properties of the additive , and on the categories of the food in which the additive will be used .
	manualset3
129463	7	405961	13	NULL	NULL	0	NULL	functional properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A method that may be applied for this purpose is the Danish Budget Method which estimates the maximum amount of the additive that may be added to the food based on the functional properties of the additive , and on the categories of the food in which the additive will be used .
	manualset3
129464	8	405961	13	NULL	NULL	0	NULL	additive	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A method that may be applied for this purpose is the Danish Budget Method which estimates the maximum amount of the additive that may be added to the food based on the functional properties of the additive , and on the categories of the food in which the additive will be used .
	manualset3
129465	9	405961	13	NULL	NULL	0	NULL	categories	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A method that may be applied for this purpose is the Danish Budget Method which estimates the maximum amount of the additive that may be added to the food based on the functional properties of the additive , and on the categories of the food in which the additive will be used .
	manualset3
129466	10	405961	13	NULL	NULL	0	NULL	food	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A method that may be applied for this purpose is the Danish Budget Method which estimates the maximum amount of the additive that may be added to the food based on the functional properties of the additive , and on the categories of the food in which the additive will be used .
	manualset3
129467	11	405961	13	NULL	NULL	0	NULL	additive	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A method that may be applied for this purpose is the Danish Budget Method which estimates the maximum amount of the additive that may be added to the food based on the functional properties of the additive , and on the categories of the food in which the additive will be used .
	manualset3
129468	1	405962	13	NULL	NULL	0	NULL	Recalcitrant lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recalcitrant lesions of pemphigus foliaceous at a surgical site : successful treatment with tacrolimus 0.1 % ointment .
	manualset3
129469	2	405962	13	NULL	NULL	0	NULL	pemphigus foliaceous	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Recalcitrant lesions of pemphigus foliaceous at a surgical site : successful treatment with tacrolimus 0.1 % ointment .
	manualset3
129470	3	405962	13	NULL	NULL	0	NULL	surgical site	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Recalcitrant lesions of pemphigus foliaceous at a surgical site : successful treatment with tacrolimus 0.1 % ointment .
	manualset3
129574	4	405962	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recalcitrant lesions of pemphigus foliaceous at a surgical site : successful treatment with tacrolimus 0.1 % ointment .
	manualset3
129575	5	405962	13	NULL	NULL	0	NULL	tacrolimus 0.1 % ointment 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Recalcitrant lesions of pemphigus foliaceous at a surgical site : successful treatment with tacrolimus 0.1 % ointment .
	manualset3
129576	1	405963	13	NULL	NULL	0	NULL	Australian experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent Australian experience with hemopoietic stem and progenitor cell expansion .
	manualset3
129577	2	405963	13	NULL	NULL	0	NULL	hemopoietic stem cell expansion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent Australian experience with hemopoietic stem and progenitor cell expansion .
	manualset3
129578	3	405963	13	NULL	NULL	0	NULL	hemopoietic progenitor cell expansion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent Australian experience with hemopoietic stem and progenitor cell expansion .
	manualset3
129579	1	405964	13	NULL	NULL	0	NULL	advances 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in DECT focus on noise reduction techniques ( S. Richard and J. H. Siewerdsen , Med .
	manualset3
129580	2	405964	13	NULL	NULL	0	NULL	DECT focus	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in DECT focus on noise reduction techniques ( S. Richard and J. H. Siewerdsen , Med .
	manualset3
129581	3	405964	13	NULL	NULL	0	NULL	noise reduction techniques	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in DECT focus on noise reduction techniques ( S. Richard and J. H. Siewerdsen , Med .
	manualset3
129582	4	405964	13	NULL	NULL	0	NULL	S. Richard	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in DECT focus on noise reduction techniques ( S. Richard and J. H. Siewerdsen , Med .
	manualset3
129583	5	405964	13	NULL	NULL	0	NULL	J. H. Siewerdsen	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in DECT focus on noise reduction techniques ( S. Richard and J. H. Siewerdsen , Med .
	manualset3
129584	1	405965	13	NULL	NULL	0	NULL	advances 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in medical treatment make it even more important that accurate information is available regarding outcome of SCT in relevant patient populations in order to guide informed decisions regarding the most appropriate treatment for individual thalassemia patients .
	manualset3
129585	2	405965	13	NULL	NULL	0	NULL	medical treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in medical treatment make it even more important that accurate information is available regarding outcome of SCT in relevant patient populations in order to guide informed decisions regarding the most appropriate treatment for individual thalassemia patients .
	manualset3
129586	3	405965	13	NULL	NULL	NULL	NULL	information	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Recent advances in medical treatment make it even more important that accurate information is available regarding outcome of SCT in relevant patient populations in order to guide informed decisions regarding the most appropriate treatment for individual thalassemia patients .
	manualset3
129587	4	405965	13	NULL	NULL	0	NULL	outcome of SCT	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in medical treatment make it even more important that accurate information is available regarding outcome of SCT in relevant patient populations in order to guide informed decisions regarding the most appropriate treatment for individual thalassemia patients .
	manualset3
129588	5	405965	13	NULL	NULL	0	NULL	patient populations 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in medical treatment make it even more important that accurate information is available regarding outcome of SCT in relevant patient populations in order to guide informed decisions regarding the most appropriate treatment for individual thalassemia patients .
	manualset3
129589	6	405965	13	NULL	NULL	0	NULL	decisions	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in medical treatment make it even more important that accurate information is available regarding outcome of SCT in relevant patient populations in order to guide informed decisions regarding the most appropriate treatment for individual thalassemia patients .
	manualset3
129590	7	405965	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in medical treatment make it even more important that accurate information is available regarding outcome of SCT in relevant patient populations in order to guide informed decisions regarding the most appropriate treatment for individual thalassemia patients .
	manualset3
129591	8	405965	13	NULL	NULL	0	NULL	individual thalassemia patients	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in medical treatment make it even more important that accurate information is available regarding outcome of SCT in relevant patient populations in order to guide informed decisions regarding the most appropriate treatment for individual thalassemia patients .
	manualset3
129592	1	405966	13	NULL	NULL	0	NULL	Recent advances	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in the convergence of the biological , chemical , physical , and engineering sciences have opened new avenues of research into the interfacing of diverse biological moieties with inanimate platforms .
	manualset3
129593	2	405966	13	NULL	NULL	0	NULL	convergence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in the convergence of the biological , chemical , physical , and engineering sciences have opened new avenues of research into the interfacing of diverse biological moieties with inanimate platforms .
	manualset3
129594	3	405966	13	NULL	NULL	0	NULL	biological sciences 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in the convergence of the biological , chemical , physical , and engineering sciences have opened new avenues of research into the interfacing of diverse biological moieties with inanimate platforms .
	manualset3
129595	4	405966	13	NULL	NULL	0	NULL	chemical sciences	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in the convergence of the biological , chemical , physical , and engineering sciences have opened new avenues of research into the interfacing of diverse biological moieties with inanimate platforms .
	manualset3
129596	5	405966	13	NULL	NULL	0	NULL	physical 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in the convergence of the biological , chemical , physical , and engineering sciences have opened new avenues of research into the interfacing of diverse biological moieties with inanimate platforms .
	manualset3
129597	6	405966	13	NULL	NULL	0	NULL	engineering sciences	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in the convergence of the biological , chemical , physical , and engineering sciences have opened new avenues of research into the interfacing of diverse biological moieties with inanimate platforms .
	manualset3
129598	7	405966	13	NULL	NULL	0	NULL	new avenues	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in the convergence of the biological , chemical , physical , and engineering sciences have opened new avenues of research into the interfacing of diverse biological moieties with inanimate platforms .
	manualset3
129599	8	405966	13	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in the convergence of the biological , chemical , physical , and engineering sciences have opened new avenues of research into the interfacing of diverse biological moieties with inanimate platforms .
	manualset3
129600	9	405966	13	NULL	NULL	0	NULL	interfacing 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in the convergence of the biological , chemical , physical , and engineering sciences have opened new avenues of research into the interfacing of diverse biological moieties with inanimate platforms .
	manualset3
129601	10	405966	13	NULL	NULL	NULL	NULL	biological moieties	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Recent advances in the convergence of the biological , chemical , physical , and engineering sciences have opened new avenues of research into the interfacing of diverse biological moieties with inanimate platforms .
	manualset3
129602	11	405966	13	NULL	NULL	0	NULL	inanimate platforms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in the convergence of the biological , chemical , physical , and engineering sciences have opened new avenues of research into the interfacing of diverse biological moieties with inanimate platforms .
	manualset3
129603	1	405967	13	NULL	NULL	0	NULL	Recent advances	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in the solid phase synthesis of drug-like heterocyclic small molecules .
	manualset3
129604	2	405967	13	NULL	NULL	0	NULL	solid phase synthesis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in the solid phase synthesis of drug-like heterocyclic small molecules .
	manualset3
129605	3	405967	13	NULL	NULL	0	NULL	drug-like heterocyclic small molecules	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in the solid phase synthesis of drug-like heterocyclic small molecules .
	manualset3
129606	1	405968	13	NULL	NULL	0	NULL	method 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A method to accomplish a 1 , 4-addition reaction of bulky nucleophiles to enones and subsequent formation of reactive enolates .
	manualset3
129607	2	405968	13	NULL	NULL	0	NULL	1 , 4-addition reaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A method to accomplish a 1 , 4-addition reaction of bulky nucleophiles to enones and subsequent formation of reactive enolates .
	manualset3
129608	3	405968	13	NULL	NULL	0	NULL	bulky nucleophiles 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A method to accomplish a 1 , 4-addition reaction of bulky nucleophiles to enones and subsequent formation of reactive enolates .
	manualset3
129609	4	405968	13	NULL	NULL	0	NULL	enones	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A method to accomplish a 1 , 4-addition reaction of bulky nucleophiles to enones and subsequent formation of reactive enolates .
	manualset3
129610	5	405968	13	NULL	NULL	0	NULL	formation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A method to accomplish a 1 , 4-addition reaction of bulky nucleophiles to enones and subsequent formation of reactive enolates .
	manualset3
129611	6	405968	13	NULL	NULL	0	NULL	reactive enolates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A method to accomplish a 1 , 4-addition reaction of bulky nucleophiles to enones and subsequent formation of reactive enolates .
	manualset3
129612	1	405969	13	NULL	NULL	0	NULL	Recent advances 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in the study on resveratrol .
	manualset3
129613	2	405969	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in the study on resveratrol .
	manualset3
129614	3	405969	13	NULL	NULL	0	NULL	resveratrol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in the study on resveratrol .
	manualset3
129615	1	405970	13	NULL	NULL	0	NULL	Recent analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent analyses tried to explain the meaning of the Brief Psychiatric Rating Scale total score ( BPRS ) and its percentage change from baseline by equipercentile linking with the Clinical Global Impression Scale ( CGI ) .
	manualset3
129616	2	405970	13	NULL	NULL	0	NULL	meaning 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent analyses tried to explain the meaning of the Brief Psychiatric Rating Scale total score ( BPRS ) and its percentage change from baseline by equipercentile linking with the Clinical Global Impression Scale ( CGI ) .
	manualset3
129617	3	405970	13	NULL	NULL	0	NULL	Brief Psychiatric Rating Scale total score ( BPRS )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent analyses tried to explain the meaning of the Brief Psychiatric Rating Scale total score ( BPRS ) and its percentage change from baseline by equipercentile linking with the Clinical Global Impression Scale ( CGI ) .
	manualset3
129618	4	405970	13	NULL	NULL	0	NULL	percentage change	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent analyses tried to explain the meaning of the Brief Psychiatric Rating Scale total score ( BPRS ) and its percentage change from baseline by equipercentile linking with the Clinical Global Impression Scale ( CGI ) .
	manualset3
129619	5	405970	13	NULL	NULL	0	NULL	baseline	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent analyses tried to explain the meaning of the Brief Psychiatric Rating Scale total score ( BPRS ) and its percentage change from baseline by equipercentile linking with the Clinical Global Impression Scale ( CGI ) .
	manualset3
129620	6	405970	13	NULL	NULL	0	NULL	equipercentile 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent analyses tried to explain the meaning of the Brief Psychiatric Rating Scale total score ( BPRS ) and its percentage change from baseline by equipercentile linking with the Clinical Global Impression Scale ( CGI ) .
	manualset3
129621	7	405970	13	NULL	NULL	0	NULL	Clinical Global Impression Scale ( CGI ) 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent analyses tried to explain the meaning of the Brief Psychiatric Rating Scale total score ( BPRS ) and its percentage change from baseline by equipercentile linking with the Clinical Global Impression Scale ( CGI ) .
	manualset3
129622	1	405971	13	NULL	NULL	0	NULL	anatomic studies 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent anatomic studies of human subcortical regions , limited to the striatum , have failed to show a size asymmetry .
	manualset3
129623	2	405971	13	NULL	NULL	0	NULL	human subcortical regions 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent anatomic studies of human subcortical regions , limited to the striatum , have failed to show a size asymmetry .
	manualset3
129624	3	405971	13	NULL	NULL	0	NULL	striatum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent anatomic studies of human subcortical regions , limited to the striatum , have failed to show a size asymmetry .
	manualset3
129625	4	405971	13	NULL	NULL	NULL	NULL	size asymmetry 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Recent anatomic studies of human subcortical regions , limited to the striatum , have failed to show a size asymmetry .
	manualset3
129626	1	405972	13	NULL	NULL	0	NULL	articles 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent articles and reports of research indicate that application of human factor principles and procedures to : ( 1 ) develop appropriate display formats , ( 2 ) consider the total avionics suite as an integrated system , and ( 3 ) simplify or summarize related data will significantly improve total aircraft performance .
	manualset3
129627	2	405972	13	NULL	NULL	0	NULL	reports	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent articles and reports of research indicate that application of human factor principles and procedures to : ( 1 ) develop appropriate display formats , ( 2 ) consider the total avionics suite as an integrated system , and ( 3 ) simplify or summarize related data will significantly improve total aircraft performance .
	manualset3
129628	3	405972	13	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent articles and reports of research indicate that application of human factor principles and procedures to : ( 1 ) develop appropriate display formats , ( 2 ) consider the total avionics suite as an integrated system , and ( 3 ) simplify or summarize related data will significantly improve total aircraft performance .
	manualset3
129629	4	405972	13	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent articles and reports of research indicate that application of human factor principles and procedures to : ( 1 ) develop appropriate display formats , ( 2 ) consider the total avionics suite as an integrated system , and ( 3 ) simplify or summarize related data will significantly improve total aircraft performance .
	manualset3
129630	5	405972	13	NULL	NULL	0	NULL	human factor principles	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent articles and reports of research indicate that application of human factor principles and procedures to : ( 1 ) develop appropriate display formats , ( 2 ) consider the total avionics suite as an integrated system , and ( 3 ) simplify or summarize related data will significantly improve total aircraft performance .
	manualset3
129631	6	405972	13	NULL	NULL	0	NULL	procedures	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent articles and reports of research indicate that application of human factor principles and procedures to : ( 1 ) develop appropriate display formats , ( 2 ) consider the total avionics suite as an integrated system , and ( 3 ) simplify or summarize related data will significantly improve total aircraft performance .
	manualset3
129632	7	405972	13	NULL	NULL	0	NULL	display formats 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent articles and reports of research indicate that application of human factor principles and procedures to : ( 1 ) develop appropriate display formats , ( 2 ) consider the total avionics suite as an integrated system , and ( 3 ) simplify or summarize related data will significantly improve total aircraft performance .
	manualset3
129633	8	405972	13	NULL	NULL	NULL	NULL	total avionics suite	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Recent articles and reports of research indicate that application of human factor principles and procedures to : ( 1 ) develop appropriate display formats , ( 2 ) consider the total avionics suite as an integrated system , and ( 3 ) simplify or summarize related data will significantly improve total aircraft performance .
	manualset3
129634	9	405972	13	NULL	NULL	0	NULL	integrated system	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent articles and reports of research indicate that application of human factor principles and procedures to : ( 1 ) develop appropriate display formats , ( 2 ) consider the total avionics suite as an integrated system , and ( 3 ) simplify or summarize related data will significantly improve total aircraft performance .
	manualset3
129635	10	405972	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent articles and reports of research indicate that application of human factor principles and procedures to : ( 1 ) develop appropriate display formats , ( 2 ) consider the total avionics suite as an integrated system , and ( 3 ) simplify or summarize related data will significantly improve total aircraft performance .
	manualset3
129636	11	405972	13	NULL	NULL	0	NULL	total aircraft performance	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent articles and reports of research indicate that application of human factor principles and procedures to : ( 1 ) develop appropriate display formats , ( 2 ) consider the total avionics suite as an integrated system , and ( 3 ) simplify or summarize related data will significantly improve total aircraft performance .
	manualset3
129637	1	405973	13	NULL	NULL	0	NULL	behavioral research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent behavioral , neuroimaging , and neurophysiological research suggests a common representational code mediating the observation and execution of actions ; yet , the nature of this representational code is not well understood .
	manualset3
129638	2	405973	13	NULL	NULL	0	NULL	neuroimaging research 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent behavioral , neuroimaging , and neurophysiological research suggests a common representational code mediating the observation and execution of actions ; yet , the nature of this representational code is not well understood .
	manualset3
129639	3	405973	13	NULL	NULL	0	NULL	neurophysiological research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent behavioral , neuroimaging , and neurophysiological research suggests a common representational code mediating the observation and execution of actions ; yet , the nature of this representational code is not well understood .
	manualset3
129640	4	405973	13	NULL	NULL	0	NULL	representational code	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent behavioral , neuroimaging , and neurophysiological research suggests a common representational code mediating the observation and execution of actions ; yet , the nature of this representational code is not well understood .
	manualset3
129641	5	405973	13	NULL	NULL	0	NULL	observation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent behavioral , neuroimaging , and neurophysiological research suggests a common representational code mediating the observation and execution of actions ; yet , the nature of this representational code is not well understood .
	manualset3
129642	6	405973	13	NULL	NULL	0	NULL	execution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent behavioral , neuroimaging , and neurophysiological research suggests a common representational code mediating the observation and execution of actions ; yet , the nature of this representational code is not well understood .
	manualset3
129643	7	405973	13	NULL	NULL	0	NULL	actions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent behavioral , neuroimaging , and neurophysiological research suggests a common representational code mediating the observation and execution of actions ; yet , the nature of this representational code is not well understood .
	manualset3
129644	8	405973	13	NULL	NULL	0	NULL	nature 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent behavioral , neuroimaging , and neurophysiological research suggests a common representational code mediating the observation and execution of actions ; yet , the nature of this representational code is not well understood .
	manualset3
129645	9	405973	13	NULL	NULL	0	NULL	representational code 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent behavioral , neuroimaging , and neurophysiological research suggests a common representational code mediating the observation and execution of actions ; yet , the nature of this representational code is not well understood .
	manualset3
129646	1	405974	13	NULL	NULL	0	NULL	concepts	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent concepts in feline lower urinary tract disease .
	manualset3
129647	2	405974	13	NULL	NULL	0	NULL	feline lower urinary tract disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent concepts in feline lower urinary tract disease .
	manualset3
129648	1	405975	13	NULL	NULL	0	NULL	cytogenetic data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent cytogenetic data indicate that the specific changes observed in various types of ANLL may be seen in corresponding types of MT , such as t ( 15 ; 17 ) in promyelocytic transformations and abnormalities of 3q21-3q26 in megakaryoblastic transformations .
	manualset3
129649	2	405975	13	NULL	NULL	0	NULL	changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent cytogenetic data indicate that the specific changes observed in various types of ANLL may be seen in corresponding types of MT , such as t ( 15 ; 17 ) in promyelocytic transformations and abnormalities of 3q21-3q26 in megakaryoblastic transformations .
	manualset3
129650	3	405975	13	NULL	NULL	0	NULL	various types of ANLL 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent cytogenetic data indicate that the specific changes observed in various types of ANLL may be seen in corresponding types of MT , such as t ( 15 ; 17 ) in promyelocytic transformations and abnormalities of 3q21-3q26 in megakaryoblastic transformations .
	manualset3
129651	4	405975	13	NULL	NULL	0	NULL	types of MT	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent cytogenetic data indicate that the specific changes observed in various types of ANLL may be seen in corresponding types of MT , such as t ( 15 ; 17 ) in promyelocytic transformations and abnormalities of 3q21-3q26 in megakaryoblastic transformations .
	manualset3
129652	5	405975	13	NULL	NULL	0	NULL	t ( 15 ; 17 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent cytogenetic data indicate that the specific changes observed in various types of ANLL may be seen in corresponding types of MT , such as t ( 15 ; 17 ) in promyelocytic transformations and abnormalities of 3q21-3q26 in megakaryoblastic transformations .
	manualset3
129653	6	405975	13	NULL	NULL	0	NULL	promyelocytic transformations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent cytogenetic data indicate that the specific changes observed in various types of ANLL may be seen in corresponding types of MT , such as t ( 15 ; 17 ) in promyelocytic transformations and abnormalities of 3q21-3q26 in megakaryoblastic transformations .
	manualset3
129654	7	405975	13	NULL	NULL	0	NULL	abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent cytogenetic data indicate that the specific changes observed in various types of ANLL may be seen in corresponding types of MT , such as t ( 15 ; 17 ) in promyelocytic transformations and abnormalities of 3q21-3q26 in megakaryoblastic transformations .
	manualset3
129655	8	405975	13	NULL	NULL	0	NULL	3q21-3q26	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent cytogenetic data indicate that the specific changes observed in various types of ANLL may be seen in corresponding types of MT , such as t ( 15 ; 17 ) in promyelocytic transformations and abnormalities of 3q21-3q26 in megakaryoblastic transformations .
	manualset3
129656	9	405975	13	NULL	NULL	NULL	NULL	megakaryoblastic transformations	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Recent cytogenetic data indicate that the specific changes observed in various types of ANLL may be seen in corresponding types of MT , such as t ( 15 ; 17 ) in promyelocytic transformations and abnormalities of 3q21-3q26 in megakaryoblastic transformations .
	manualset3
129657	1	405976	13	NULL	NULL	0	NULL	developments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent developments in evolution theory ( based on an analysis of Cambrian fossils in Canada 's Burgess Shale quarry ) suggest that evolution passes , at times , through innovative cycles of progress -- when diversification of design leads to perfection of form -- with the concomitant production of many unsuccessful models .
	manualset3
129658	2	405976	13	NULL	NULL	0	NULL	evolution theory	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent developments in evolution theory ( based on an analysis of Cambrian fossils in Canada 's Burgess Shale quarry ) suggest that evolution passes , at times , through innovative cycles of progress -- when diversification of design leads to perfection of form -- with the concomitant production of many unsuccessful models .
	manualset3
129659	3	405976	13	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent developments in evolution theory ( based on an analysis of Cambrian fossils in Canada 's Burgess Shale quarry ) suggest that evolution passes , at times , through innovative cycles of progress -- when diversification of design leads to perfection of form -- with the concomitant production of many unsuccessful models .
	manualset3
129660	4	405976	13	NULL	NULL	0	NULL	Cambrian fossils	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent developments in evolution theory ( based on an analysis of Cambrian fossils in Canada 's Burgess Shale quarry ) suggest that evolution passes , at times , through innovative cycles of progress -- when diversification of design leads to perfection of form -- with the concomitant production of many unsuccessful models .
	manualset3
129661	5	405976	13	NULL	NULL	0	NULL	Canada 's Burgess Shale quarry	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent developments in evolution theory ( based on an analysis of Cambrian fossils in Canada 's Burgess Shale quarry ) suggest that evolution passes , at times , through innovative cycles of progress -- when diversification of design leads to perfection of form -- with the concomitant production of many unsuccessful models .
	manualset3
129662	6	405976	13	NULL	NULL	0	NULL	evolution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent developments in evolution theory ( based on an analysis of Cambrian fossils in Canada 's Burgess Shale quarry ) suggest that evolution passes , at times , through innovative cycles of progress -- when diversification of design leads to perfection of form -- with the concomitant production of many unsuccessful models .
	manualset3
129663	7	405976	13	NULL	NULL	0	NULL	innovative cycles 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent developments in evolution theory ( based on an analysis of Cambrian fossils in Canada 's Burgess Shale quarry ) suggest that evolution passes , at times , through innovative cycles of progress -- when diversification of design leads to perfection of form -- with the concomitant production of many unsuccessful models .
	manualset3
129664	8	405976	13	NULL	NULL	0	NULL	progress	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent developments in evolution theory ( based on an analysis of Cambrian fossils in Canada 's Burgess Shale quarry ) suggest that evolution passes , at times , through innovative cycles of progress -- when diversification of design leads to perfection of form -- with the concomitant production of many unsuccessful models .
	manualset3
129665	9	405976	13	NULL	NULL	0	NULL	diversification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent developments in evolution theory ( based on an analysis of Cambrian fossils in Canada 's Burgess Shale quarry ) suggest that evolution passes , at times , through innovative cycles of progress -- when diversification of design leads to perfection of form -- with the concomitant production of many unsuccessful models .
	manualset3
129666	10	405976	13	NULL	NULL	0	NULL	design	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent developments in evolution theory ( based on an analysis of Cambrian fossils in Canada 's Burgess Shale quarry ) suggest that evolution passes , at times , through innovative cycles of progress -- when diversification of design leads to perfection of form -- with the concomitant production of many unsuccessful models .
	manualset3
129667	11	405976	13	NULL	NULL	0	NULL	perfection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent developments in evolution theory ( based on an analysis of Cambrian fossils in Canada 's Burgess Shale quarry ) suggest that evolution passes , at times , through innovative cycles of progress -- when diversification of design leads to perfection of form -- with the concomitant production of many unsuccessful models .
	manualset3
129668	12	405976	13	NULL	NULL	0	NULL	form	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent developments in evolution theory ( based on an analysis of Cambrian fossils in Canada 's Burgess Shale quarry ) suggest that evolution passes , at times , through innovative cycles of progress -- when diversification of design leads to perfection of form -- with the concomitant production of many unsuccessful models .
	manualset3
129669	13	405976	13	NULL	NULL	0	NULL	production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent developments in evolution theory ( based on an analysis of Cambrian fossils in Canada 's Burgess Shale quarry ) suggest that evolution passes , at times , through innovative cycles of progress -- when diversification of design leads to perfection of form -- with the concomitant production of many unsuccessful models .
	manualset3
129670	14	405976	13	NULL	NULL	0	NULL	models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent developments in evolution theory ( based on an analysis of Cambrian fossils in Canada 's Burgess Shale quarry ) suggest that evolution passes , at times , through innovative cycles of progress -- when diversification of design leads to perfection of form -- with the concomitant production of many unsuccessful models .
	manualset3
129671	1	405977	13	NULL	NULL	0	NULL	method 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A method to protect the hips during falls could effectively reduce the incidence of hip fractures .
	manualset3
129672	2	405977	13	NULL	NULL	0	NULL	hips	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A method to protect the hips during falls could effectively reduce the incidence of hip fractures .
	manualset3
129673	3	405977	13	NULL	NULL	0	NULL	incidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A method to protect the hips during falls could effectively reduce the incidence of hip fractures .
	manualset3
129674	4	405977	13	NULL	NULL	0	NULL	hip fractures 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A method to protect the hips during falls could effectively reduce the incidence of hip fractures .
	manualset3
129675	1	405978	13	NULL	NULL	0	NULL	discoveries	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent discoveries in kidney research have given new insights into the molecular make-up of the glomerular filter and mechanisms of permselectivity .
	manualset3
129676	2	405978	13	NULL	NULL	0	NULL	kidney research 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent discoveries in kidney research have given new insights into the molecular make-up of the glomerular filter and mechanisms of permselectivity .
	manualset3
129677	3	405978	13	NULL	NULL	NULL	NULL	new insights 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Recent discoveries in kidney research have given new insights into the molecular make-up of the glomerular filter and mechanisms of permselectivity .
	manualset3
129679	5	405978	13	NULL	NULL	NULL	NULL	glomerular filter	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Recent discoveries in kidney research have given new insights into the molecular make-up of the glomerular filter and mechanisms of permselectivity .
	manualset3
129680	6	405978	13	NULL	NULL	0	NULL	mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent discoveries in kidney research have given new insights into the molecular make-up of the glomerular filter and mechanisms of permselectivity .
	manualset3
129681	7	405978	13	NULL	NULL	0	NULL	permselectivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent discoveries in kidney research have given new insights into the molecular make-up of the glomerular filter and mechanisms of permselectivity .
	manualset3
129678	1	405979	13	NULL	NULL	NULL	NULL	evidence	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Recent evidence implicates a critical role for redox regulation and thiol balance in pathways that control myeloproliferation , hematopoietic progenitor cell mobilization , and immune response .
	manualset3
129682	2	405979	13	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent evidence implicates a critical role for redox regulation and thiol balance in pathways that control myeloproliferation , hematopoietic progenitor cell mobilization , and immune response .
	manualset3
129683	3	405979	13	NULL	NULL	0	NULL	redox regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent evidence implicates a critical role for redox regulation and thiol balance in pathways that control myeloproliferation , hematopoietic progenitor cell mobilization , and immune response .
	manualset3
129684	4	405979	13	NULL	NULL	0	NULL	thiol balance	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent evidence implicates a critical role for redox regulation and thiol balance in pathways that control myeloproliferation , hematopoietic progenitor cell mobilization , and immune response .
	manualset3
129685	5	405979	13	NULL	NULL	0	NULL	pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent evidence implicates a critical role for redox regulation and thiol balance in pathways that control myeloproliferation , hematopoietic progenitor cell mobilization , and immune response .
	manualset3
129686	6	405979	13	NULL	NULL	0	NULL	myeloproliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent evidence implicates a critical role for redox regulation and thiol balance in pathways that control myeloproliferation , hematopoietic progenitor cell mobilization , and immune response .
	manualset3
129687	7	405979	13	NULL	NULL	0	NULL	hematopoietic progenitor cell mobilization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent evidence implicates a critical role for redox regulation and thiol balance in pathways that control myeloproliferation , hematopoietic progenitor cell mobilization , and immune response .
	manualset3
129688	8	405979	13	NULL	NULL	0	NULL	immune response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent evidence implicates a critical role for redox regulation and thiol balance in pathways that control myeloproliferation , hematopoietic progenitor cell mobilization , and immune response .
	manualset3
129689	1	405980	13	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent evidence suggests that the molecular machinery of RNA interference may function as an important host defense against TEs .
	manualset3
129690	2	405980	13	NULL	NULL	0	NULL	molecular machinery 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent evidence suggests that the molecular machinery of RNA interference may function as an important host defense against TEs .
	manualset3
129691	3	405980	13	NULL	NULL	0	NULL	RNA interference	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent evidence suggests that the molecular machinery of RNA interference may function as an important host defense against TEs .
	manualset3
129692	4	405980	13	NULL	NULL	0	NULL	host defense 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent evidence suggests that the molecular machinery of RNA interference may function as an important host defense against TEs .
	manualset3
129693	5	405980	13	NULL	NULL	0	NULL	TEs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent evidence suggests that the molecular machinery of RNA interference may function as an important host defense against TEs .
	manualset3
129694	1	405981	13	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent evidence suggests that treatment with low-dose acetylsalicylic acid ( ASA ) started early in pregnancy could prevent preeclampsia and intrauterine growth restriction ( IUGR ) , two complications involving placental dysfunction .
	manualset3
129695	2	405981	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent evidence suggests that treatment with low-dose acetylsalicylic acid ( ASA ) started early in pregnancy could prevent preeclampsia and intrauterine growth restriction ( IUGR ) , two complications involving placental dysfunction .
	manualset3
129696	3	405981	13	NULL	NULL	0	NULL	low-dose acetylsalicylic acid ( ASA )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent evidence suggests that treatment with low-dose acetylsalicylic acid ( ASA ) started early in pregnancy could prevent preeclampsia and intrauterine growth restriction ( IUGR ) , two complications involving placental dysfunction .
	manualset3
129697	4	405981	13	NULL	NULL	0	NULL	pregnancy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent evidence suggests that treatment with low-dose acetylsalicylic acid ( ASA ) started early in pregnancy could prevent preeclampsia and intrauterine growth restriction ( IUGR ) , two complications involving placental dysfunction .
	manualset3
129698	5	405981	13	NULL	NULL	0	NULL	preeclampsia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent evidence suggests that treatment with low-dose acetylsalicylic acid ( ASA ) started early in pregnancy could prevent preeclampsia and intrauterine growth restriction ( IUGR ) , two complications involving placental dysfunction .
	manualset3
129699	6	405981	13	NULL	NULL	0	NULL	intrauterine growth restriction ( IUGR ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent evidence suggests that treatment with low-dose acetylsalicylic acid ( ASA ) started early in pregnancy could prevent preeclampsia and intrauterine growth restriction ( IUGR ) , two complications involving placental dysfunction .
	manualset3
129700	7	405981	13	NULL	NULL	0	NULL	two complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent evidence suggests that treatment with low-dose acetylsalicylic acid ( ASA ) started early in pregnancy could prevent preeclampsia and intrauterine growth restriction ( IUGR ) , two complications involving placental dysfunction .
	manualset3
129701	8	405981	13	NULL	NULL	0	NULL	placental dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent evidence suggests that treatment with low-dose acetylsalicylic acid ( ASA ) started early in pregnancy could prevent preeclampsia and intrauterine growth restriction ( IUGR ) , two complications involving placental dysfunction .
	manualset3
129702	1	405982	13	NULL	NULL	0	NULL	experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent experiments have demonstrated the effectiveness of members of the neurotrophin family of growth factors in supporting the survival of primary auditory neurons following ototoxic trauma .
	manualset3
129703	2	405982	13	NULL	NULL	0	NULL	effectiveness	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent experiments have demonstrated the effectiveness of members of the neurotrophin family of growth factors in supporting the survival of primary auditory neurons following ototoxic trauma .
	manualset3
129704	3	405982	13	NULL	NULL	0	NULL	members 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent experiments have demonstrated the effectiveness of members of the neurotrophin family of growth factors in supporting the survival of primary auditory neurons following ototoxic trauma .
	manualset3
129705	4	405982	13	NULL	NULL	0	NULL	neurotrophin family of growth factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent experiments have demonstrated the effectiveness of members of the neurotrophin family of growth factors in supporting the survival of primary auditory neurons following ototoxic trauma .
	manualset3
129706	5	405982	13	NULL	NULL	0	NULL	survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent experiments have demonstrated the effectiveness of members of the neurotrophin family of growth factors in supporting the survival of primary auditory neurons following ototoxic trauma .
	manualset3
129707	6	405982	13	NULL	NULL	0	NULL	primary auditory neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent experiments have demonstrated the effectiveness of members of the neurotrophin family of growth factors in supporting the survival of primary auditory neurons following ototoxic trauma .
	manualset3
129708	7	405982	13	NULL	NULL	0	NULL	ototoxic trauma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent experiments have demonstrated the effectiveness of members of the neurotrophin family of growth factors in supporting the survival of primary auditory neurons following ototoxic trauma .
	manualset3
129709	1	405983	13	NULL	NULL	0	NULL	findings	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent findings that TAFs may not be globally required for activator-dependent transcription in vivo and in vitro and that both TAF-dependent and TAF-independent promoters are found in yeast suggest that transcriptional activation can occur through at least two different pathways , depending on the presence or absence of TAFs .
	manualset3
129710	2	405983	13	NULL	NULL	0	NULL	TAFs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent findings that TAFs may not be globally required for activator-dependent transcription in vivo and in vitro and that both TAF-dependent and TAF-independent promoters are found in yeast suggest that transcriptional activation can occur through at least two different pathways , depending on the presence or absence of TAFs .
	manualset3
129711	3	405983	13	NULL	NULL	0	NULL	transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent findings that TAFs may not be globally required for activator-dependent transcription in vivo and in vitro and that both TAF-dependent and TAF-independent promoters are found in yeast suggest that transcriptional activation can occur through at least two different pathways , depending on the presence or absence of TAFs .
	manualset3
129712	4	405983	13	NULL	NULL	0	NULL	TAF-dependent promoters	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent findings that TAFs may not be globally required for activator-dependent transcription in vivo and in vitro and that both TAF-dependent and TAF-independent promoters are found in yeast suggest that transcriptional activation can occur through at least two different pathways , depending on the presence or absence of TAFs .
	manualset3
129713	5	405983	13	NULL	NULL	0	NULL	TAF-independent promoters	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent findings that TAFs may not be globally required for activator-dependent transcription in vivo and in vitro and that both TAF-dependent and TAF-independent promoters are found in yeast suggest that transcriptional activation can occur through at least two different pathways , depending on the presence or absence of TAFs .
	manualset3
129714	6	405983	13	NULL	NULL	0	NULL	yeast	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent findings that TAFs may not be globally required for activator-dependent transcription in vivo and in vitro and that both TAF-dependent and TAF-independent promoters are found in yeast suggest that transcriptional activation can occur through at least two different pathways , depending on the presence or absence of TAFs .
	manualset3
129715	7	405983	13	NULL	NULL	0	NULL	transcriptional activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent findings that TAFs may not be globally required for activator-dependent transcription in vivo and in vitro and that both TAF-dependent and TAF-independent promoters are found in yeast suggest that transcriptional activation can occur through at least two different pathways , depending on the presence or absence of TAFs .
	manualset3
129716	8	405983	13	NULL	NULL	0	NULL	two different pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent findings that TAFs may not be globally required for activator-dependent transcription in vivo and in vitro and that both TAF-dependent and TAF-independent promoters are found in yeast suggest that transcriptional activation can occur through at least two different pathways , depending on the presence or absence of TAFs .
	manualset3
129717	9	405983	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent findings that TAFs may not be globally required for activator-dependent transcription in vivo and in vitro and that both TAF-dependent and TAF-independent promoters are found in yeast suggest that transcriptional activation can occur through at least two different pathways , depending on the presence or absence of TAFs .
	manualset3
129718	10	405983	13	NULL	NULL	0	NULL	absence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent findings that TAFs may not be globally required for activator-dependent transcription in vivo and in vitro and that both TAF-dependent and TAF-independent promoters are found in yeast suggest that transcriptional activation can occur through at least two different pathways , depending on the presence or absence of TAFs .
	manualset3
129719	11	405983	13	NULL	NULL	0	NULL	TAFs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent findings that TAFs may not be globally required for activator-dependent transcription in vivo and in vitro and that both TAF-dependent and TAF-independent promoters are found in yeast suggest that transcriptional activation can occur through at least two different pathways , depending on the presence or absence of TAFs .
	manualset3
129720	1	405984	13	NULL	NULL	0	NULL	investigations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent investigations , however , have indicated that nitrate-mediated benefit to patients with CHF may be limited by resistance to their hemodynamic effects seen in many patients and by early development of tolerance .
	manualset3
129721	2	405984	13	NULL	NULL	0	NULL	nitrate-mediated benefit	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent investigations , however , have indicated that nitrate-mediated benefit to patients with CHF may be limited by resistance to their hemodynamic effects seen in many patients and by early development of tolerance .
	manualset3
129722	3	405984	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent investigations , however , have indicated that nitrate-mediated benefit to patients with CHF may be limited by resistance to their hemodynamic effects seen in many patients and by early development of tolerance .
	manualset3
129723	4	405984	13	NULL	NULL	0	NULL	CHF 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent investigations , however , have indicated that nitrate-mediated benefit to patients with CHF may be limited by resistance to their hemodynamic effects seen in many patients and by early development of tolerance .
	manualset3
129724	5	405984	13	NULL	NULL	0	NULL	resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent investigations , however , have indicated that nitrate-mediated benefit to patients with CHF may be limited by resistance to their hemodynamic effects seen in many patients and by early development of tolerance .
	manualset3
129725	6	405984	13	NULL	NULL	0	NULL	hemodynamic effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent investigations , however , have indicated that nitrate-mediated benefit to patients with CHF may be limited by resistance to their hemodynamic effects seen in many patients and by early development of tolerance .
	manualset3
129726	7	405984	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent investigations , however , have indicated that nitrate-mediated benefit to patients with CHF may be limited by resistance to their hemodynamic effects seen in many patients and by early development of tolerance .
	manualset3
129727	8	405984	13	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent investigations , however , have indicated that nitrate-mediated benefit to patients with CHF may be limited by resistance to their hemodynamic effects seen in many patients and by early development of tolerance .
	manualset3
129728	9	405984	13	NULL	NULL	0	NULL	tolerance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent investigations , however , have indicated that nitrate-mediated benefit to patients with CHF may be limited by resistance to their hemodynamic effects seen in many patients and by early development of tolerance .
	manualset3
129729	1	405985	13	NULL	NULL	0	NULL	investigations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent investigations designate this signaling pathway as one of the primary targets of viral proteins after infection .
	manualset3
129730	2	405985	13	NULL	NULL	0	NULL	signaling pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent investigations designate this signaling pathway as one of the primary targets of viral proteins after infection .
	manualset3
129731	3	405985	13	NULL	NULL	0	NULL	primary targets 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent investigations designate this signaling pathway as one of the primary targets of viral proteins after infection .
	manualset3
129732	4	405985	13	NULL	NULL	0	NULL	viral proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent investigations designate this signaling pathway as one of the primary targets of viral proteins after infection .
	manualset3
129733	5	405985	13	NULL	NULL	0	NULL	infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent investigations designate this signaling pathway as one of the primary targets of viral proteins after infection .
	manualset3
129734	1	405986	13	NULL	NULL	0	NULL	methodology	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A methodology for estimating health benefits of electricity generation using renewable technologies .
	manualset3
129735	2	405986	13	NULL	NULL	0	NULL	health benefits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A methodology for estimating health benefits of electricity generation using renewable technologies .
	manualset3
129736	3	405986	13	NULL	NULL	0	NULL	electricity generation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A methodology for estimating health benefits of electricity generation using renewable technologies .
	manualset3
129737	4	405986	13	NULL	NULL	0	NULL	renewable technologies	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A methodology for estimating health benefits of electricity generation using renewable technologies .
	manualset3
129738	1	405987	13	NULL	NULL	0	NULL	knockdown studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent knockdown studies revealed that basic transcription factors are essential not only for gene transcription but also for regulating specific gene expression .
	manualset3
129739	2	405987	13	NULL	NULL	0	NULL	basic transcription factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent knockdown studies revealed that basic transcription factors are essential not only for gene transcription but also for regulating specific gene expression .
	manualset3
129740	3	405987	13	NULL	NULL	0	NULL	gene transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent knockdown studies revealed that basic transcription factors are essential not only for gene transcription but also for regulating specific gene expression .
	manualset3
129741	4	405987	13	NULL	NULL	0	NULL	gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent knockdown studies revealed that basic transcription factors are essential not only for gene transcription but also for regulating specific gene expression .
	manualset3
129742	1	405988	13	NULL	NULL	0	NULL	progress 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent progress in the understanding of molecular biology and pathogenesis of renal cell cancer has been translated into the development of new therapeutic strategies .
	manualset3
129743	2	405988	13	NULL	NULL	0	NULL	understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent progress in the understanding of molecular biology and pathogenesis of renal cell cancer has been translated into the development of new therapeutic strategies .
	manualset3
129744	3	405988	13	NULL	NULL	NULL	NULL	molecular biology	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Recent progress in the understanding of molecular biology and pathogenesis of renal cell cancer has been translated into the development of new therapeutic strategies .
	manualset3
129745	4	405988	13	NULL	NULL	0	NULL	pathogenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent progress in the understanding of molecular biology and pathogenesis of renal cell cancer has been translated into the development of new therapeutic strategies .
	manualset3
129746	5	405988	13	NULL	NULL	0	NULL	renal cell cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent progress in the understanding of molecular biology and pathogenesis of renal cell cancer has been translated into the development of new therapeutic strategies .
	manualset3
129747	6	405988	13	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent progress in the understanding of molecular biology and pathogenesis of renal cell cancer has been translated into the development of new therapeutic strategies .
	manualset3
129748	7	405988	13	NULL	NULL	0	NULL	new therapeutic strategies	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent progress in the understanding of molecular biology and pathogenesis of renal cell cancer has been translated into the development of new therapeutic strategies .
	manualset3
129749	1	405989	13	NULL	NULL	0	NULL	progress	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent progress in understanding the oculomotor system is briefly reviewed .
	manualset3
129750	2	405989	13	NULL	NULL	0	NULL	understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent progress in understanding the oculomotor system is briefly reviewed .
	manualset3
129751	3	405989	13	NULL	NULL	0	NULL	oculomotor system	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent progress in understanding the oculomotor system is briefly reviewed .
	manualset3
129752	1	405990	13	NULL	NULL	0	NULL	reports	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent reports have revealed that DMPK gene haploinsufficiency may account for cardiac conduction defects whereas cataracts may be due to haploinsufficiency of the neighboring gene , the DM-associated homeobox protein ( DMAHP or SIX5 ) gene .
	manualset3
129753	2	405990	13	NULL	NULL	0	NULL	DMPK gene haploinsufficiency	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent reports have revealed that DMPK gene haploinsufficiency may account for cardiac conduction defects whereas cataracts may be due to haploinsufficiency of the neighboring gene , the DM-associated homeobox protein ( DMAHP or SIX5 ) gene .
	manualset3
129754	3	405990	13	NULL	NULL	0	NULL	cardiac conduction defects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent reports have revealed that DMPK gene haploinsufficiency may account for cardiac conduction defects whereas cataracts may be due to haploinsufficiency of the neighboring gene , the DM-associated homeobox protein ( DMAHP or SIX5 ) gene .
	manualset3
129755	4	405990	13	NULL	NULL	0	NULL	cataracts 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent reports have revealed that DMPK gene haploinsufficiency may account for cardiac conduction defects whereas cataracts may be due to haploinsufficiency of the neighboring gene , the DM-associated homeobox protein ( DMAHP or SIX5 ) gene .
	manualset3
129756	5	405990	13	NULL	NULL	0	NULL	haploinsufficiency	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent reports have revealed that DMPK gene haploinsufficiency may account for cardiac conduction defects whereas cataracts may be due to haploinsufficiency of the neighboring gene , the DM-associated homeobox protein ( DMAHP or SIX5 ) gene .
	manualset3
129757	6	405990	13	NULL	NULL	0	NULL	neighboring gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent reports have revealed that DMPK gene haploinsufficiency may account for cardiac conduction defects whereas cataracts may be due to haploinsufficiency of the neighboring gene , the DM-associated homeobox protein ( DMAHP or SIX5 ) gene .
	manualset3
129758	7	405990	13	NULL	NULL	0	NULL	DM-associated homeobox protein ( DMAHP or SIX5 ) gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent reports have revealed that DMPK gene haploinsufficiency may account for cardiac conduction defects whereas cataracts may be due to haploinsufficiency of the neighboring gene , the DM-associated homeobox protein ( DMAHP or SIX5 ) gene .
	manualset3
129759	1	405991	13	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent research has demonstrated an association between primary disturbances characteristic of the disease , including altered dopaminergic and glutamatergic neurotransmission , and impairments in neuronal calcium ( Ca ( 2 + ) ) homeostasis and signaling .
	manualset3
129760	2	405991	13	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent research has demonstrated an association between primary disturbances characteristic of the disease , including altered dopaminergic and glutamatergic neurotransmission , and impairments in neuronal calcium ( Ca ( 2 + ) ) homeostasis and signaling .
	manualset3
129761	3	405991	13	NULL	NULL	0	NULL	primary disturbances	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent research has demonstrated an association between primary disturbances characteristic of the disease , including altered dopaminergic and glutamatergic neurotransmission , and impairments in neuronal calcium ( Ca ( 2 + ) ) homeostasis and signaling .
	manualset3
129762	4	405991	13	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent research has demonstrated an association between primary disturbances characteristic of the disease , including altered dopaminergic and glutamatergic neurotransmission , and impairments in neuronal calcium ( Ca ( 2 + ) ) homeostasis and signaling .
	manualset3
129763	5	405991	13	NULL	NULL	0	NULL	altered dopaminergic neurotransmission	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent research has demonstrated an association between primary disturbances characteristic of the disease , including altered dopaminergic and glutamatergic neurotransmission , and impairments in neuronal calcium ( Ca ( 2 + ) ) homeostasis and signaling .
	manualset3
129764	6	405991	13	NULL	NULL	0	NULL	altered glutamatergic neurotransmission	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent research has demonstrated an association between primary disturbances characteristic of the disease , including altered dopaminergic and glutamatergic neurotransmission , and impairments in neuronal calcium ( Ca ( 2 + ) ) homeostasis and signaling .
	manualset3
129765	7	405991	13	NULL	NULL	0	NULL	impairments	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent research has demonstrated an association between primary disturbances characteristic of the disease , including altered dopaminergic and glutamatergic neurotransmission , and impairments in neuronal calcium ( Ca ( 2 + ) ) homeostasis and signaling .
	manualset3
129766	8	405991	13	NULL	NULL	0	NULL	neuronal calcium ( Ca ( 2 + ) ) homeostasis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent research has demonstrated an association between primary disturbances characteristic of the disease , including altered dopaminergic and glutamatergic neurotransmission , and impairments in neuronal calcium ( Ca ( 2 + ) ) homeostasis and signaling .
	manualset3
129767	9	405991	13	NULL	NULL	NULL	NULL	neuronal calcium ( Ca ( 2 + ) ) signaling	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Recent research has demonstrated an association between primary disturbances characteristic of the disease , including altered dopaminergic and glutamatergic neurotransmission , and impairments in neuronal calcium ( Ca ( 2 + ) ) homeostasis and signaling .
	manualset3
129768	1	405992	13	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies , primarily with mouse , rat , and chicken cells , have provided evidence to support the concept that vertebrates contain the genetic information for producing a type-C RNA tumor virus in an unexpressed form in their somatic cells as well as in their germ cells .
	manualset3
129769	2	405992	13	NULL	NULL	0	NULL	mouse cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies , primarily with mouse , rat , and chicken cells , have provided evidence to support the concept that vertebrates contain the genetic information for producing a type-C RNA tumor virus in an unexpressed form in their somatic cells as well as in their germ cells .
	manualset3
129770	3	405992	13	NULL	NULL	0	NULL	chicken cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies , primarily with mouse , rat , and chicken cells , have provided evidence to support the concept that vertebrates contain the genetic information for producing a type-C RNA tumor virus in an unexpressed form in their somatic cells as well as in their germ cells .
	manualset3
129771	4	405992	13	NULL	NULL	0	NULL	rat cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies , primarily with mouse , rat , and chicken cells , have provided evidence to support the concept that vertebrates contain the genetic information for producing a type-C RNA tumor virus in an unexpressed form in their somatic cells as well as in their germ cells .
	manualset3
129772	5	405992	13	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies , primarily with mouse , rat , and chicken cells , have provided evidence to support the concept that vertebrates contain the genetic information for producing a type-C RNA tumor virus in an unexpressed form in their somatic cells as well as in their germ cells .
	manualset3
129773	6	405992	13	NULL	NULL	0	NULL	concept	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies , primarily with mouse , rat , and chicken cells , have provided evidence to support the concept that vertebrates contain the genetic information for producing a type-C RNA tumor virus in an unexpressed form in their somatic cells as well as in their germ cells .
	manualset3
129774	7	405992	13	NULL	NULL	0	NULL	vertebrates 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies , primarily with mouse , rat , and chicken cells , have provided evidence to support the concept that vertebrates contain the genetic information for producing a type-C RNA tumor virus in an unexpressed form in their somatic cells as well as in their germ cells .
	manualset3
129775	8	405992	13	NULL	NULL	0	NULL	genetic information 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies , primarily with mouse , rat , and chicken cells , have provided evidence to support the concept that vertebrates contain the genetic information for producing a type-C RNA tumor virus in an unexpressed form in their somatic cells as well as in their germ cells .
	manualset3
129776	9	405992	13	NULL	NULL	0	NULL	type-C RNA tumor virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies , primarily with mouse , rat , and chicken cells , have provided evidence to support the concept that vertebrates contain the genetic information for producing a type-C RNA tumor virus in an unexpressed form in their somatic cells as well as in their germ cells .
	manualset3
129777	10	405992	13	NULL	NULL	0	NULL	somatic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies , primarily with mouse , rat , and chicken cells , have provided evidence to support the concept that vertebrates contain the genetic information for producing a type-C RNA tumor virus in an unexpressed form in their somatic cells as well as in their germ cells .
	manualset3
129778	11	405992	13	NULL	NULL	0	NULL	germ cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies , primarily with mouse , rat , and chicken cells , have provided evidence to support the concept that vertebrates contain the genetic information for producing a type-C RNA tumor virus in an unexpressed form in their somatic cells as well as in their germ cells .
	manualset3
129779	12	405992	13	NULL	NULL	0	NULL	unexpressed form	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies , primarily with mouse , rat , and chicken cells , have provided evidence to support the concept that vertebrates contain the genetic information for producing a type-C RNA tumor virus in an unexpressed form in their somatic cells as well as in their germ cells .
	manualset3
129780	1	405993	13	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies employing a range of animal models implicate that matrix metalloproteinases regulate multiple aspects of the neuronal development and remodeling in the brain .
	manualset3
129781	2	405993	13	NULL	NULL	0	NULL	range 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies employing a range of animal models implicate that matrix metalloproteinases regulate multiple aspects of the neuronal development and remodeling in the brain .
	manualset3
129782	3	405993	13	NULL	NULL	0	NULL	animal models 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies employing a range of animal models implicate that matrix metalloproteinases regulate multiple aspects of the neuronal development and remodeling in the brain .
	manualset3
129783	4	405993	13	NULL	NULL	0	NULL	matrix metalloproteinases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies employing a range of animal models implicate that matrix metalloproteinases regulate multiple aspects of the neuronal development and remodeling in the brain .
	manualset3
129784	5	405993	13	NULL	NULL	0	NULL	multiple aspects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies employing a range of animal models implicate that matrix metalloproteinases regulate multiple aspects of the neuronal development and remodeling in the brain .
	manualset3
129785	6	405993	13	NULL	NULL	0	NULL	neuronal development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies employing a range of animal models implicate that matrix metalloproteinases regulate multiple aspects of the neuronal development and remodeling in the brain .
	manualset3
129786	7	405993	13	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies employing a range of animal models implicate that matrix metalloproteinases regulate multiple aspects of the neuronal development and remodeling in the brain .
	manualset3
134805	8	405993	13	NULL	NULL	0	NULL	remodeling	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies employing a range of animal models implicate that matrix metalloproteinases regulate multiple aspects of the neuronal development and remodeling in the brain .
	manualset3
129787	1	405994	13	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies have identified components of a gene regulatory network that underlies PMC specification and differentiation .
	manualset3
129788	2	405994	13	NULL	NULL	NULL	NULL	components 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Recent studies have identified components of a gene regulatory network that underlies PMC specification and differentiation .
	manualset3
129789	3	405994	13	NULL	NULL	0	NULL	gene regulatory network	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies have identified components of a gene regulatory network that underlies PMC specification and differentiation .
	manualset3
129790	4	405994	13	NULL	NULL	0	NULL	PMC specification	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies have identified components of a gene regulatory network that underlies PMC specification and differentiation .
	manualset3
129791	5	405994	13	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies have identified components of a gene regulatory network that underlies PMC specification and differentiation .
	manualset3
129792	1	405995	13	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies have shown that various vasoactive peptides , in addition to eliciting a contractile response , also serve as growth factors for vascular smooth muscle ans stimulate tyrosyl phosphorylation of several endogenous proteins .
	manualset3
129793	2	405995	13	NULL	NULL	0	NULL	 various vasoactive peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies have shown that various vasoactive peptides , in addition to eliciting a contractile response , also serve as growth factors for vascular smooth muscle ans stimulate tyrosyl phosphorylation of several endogenous proteins .
	manualset3
129794	3	405995	13	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies have shown that various vasoactive peptides , in addition to eliciting a contractile response , also serve as growth factors for vascular smooth muscle ans stimulate tyrosyl phosphorylation of several endogenous proteins .
	manualset3
129795	4	405995	13	NULL	NULL	0	NULL	contractile response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies have shown that various vasoactive peptides , in addition to eliciting a contractile response , also serve as growth factors for vascular smooth muscle ans stimulate tyrosyl phosphorylation of several endogenous proteins .
	manualset3
129796	5	405995	13	NULL	NULL	0	NULL	growth factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies have shown that various vasoactive peptides , in addition to eliciting a contractile response , also serve as growth factors for vascular smooth muscle ans stimulate tyrosyl phosphorylation of several endogenous proteins .
	manualset3
129797	6	405995	13	NULL	NULL	0	NULL	vascular smooth muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies have shown that various vasoactive peptides , in addition to eliciting a contractile response , also serve as growth factors for vascular smooth muscle ans stimulate tyrosyl phosphorylation of several endogenous proteins .
	manualset3
129798	7	405995	13	NULL	NULL	0	NULL	tyrosyl phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies have shown that various vasoactive peptides , in addition to eliciting a contractile response , also serve as growth factors for vascular smooth muscle ans stimulate tyrosyl phosphorylation of several endogenous proteins .
	manualset3
129799	8	405995	13	NULL	NULL	0	NULL	several endogenous proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies have shown that various vasoactive peptides , in addition to eliciting a contractile response , also serve as growth factors for vascular smooth muscle ans stimulate tyrosyl phosphorylation of several endogenous proteins .
	manualset3
129800	1	405996	13	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies have uncovered critical molecular events underlying melanocytic transformation and melanomagenesis .
	manualset3
129801	2	405996	13	NULL	NULL	0	NULL	molecular events	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies have uncovered critical molecular events underlying melanocytic transformation and melanomagenesis .
	manualset3
129802	3	405996	13	NULL	NULL	0	NULL	melanocytic transformation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies have uncovered critical molecular events underlying melanocytic transformation and melanomagenesis .
	manualset3
129803	4	405996	13	NULL	NULL	0	NULL	melanomagenesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies have uncovered critical molecular events underlying melanocytic transformation and melanomagenesis .
	manualset3
129804	1	405997	13	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies in our laboratory demonstrating the effectiveness of rovIL-1 as an adjuvant in single and multi-component bacterial toxoid vaccines , and studies from other laboratories demonstrating the application of rbovIL-1 as an adjuvant for the response in cattle to live attenuated viral vaccines , suggest that rIL-1 may become the adjuvant of choice for diseases where protection is mediated by high levels of circulating antibody ( Ab ) .
	manualset3
129805	2	405997	13	NULL	NULL	0	NULL	laboratory	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies in our laboratory demonstrating the effectiveness of rovIL-1 as an adjuvant in single and multi-component bacterial toxoid vaccines , and studies from other laboratories demonstrating the application of rbovIL-1 as an adjuvant for the response in cattle to live attenuated viral vaccines , suggest that rIL-1 may become the adjuvant of choice for diseases where protection is mediated by high levels of circulating antibody ( Ab ) .
	manualset3
129806	3	405997	13	NULL	NULL	0	NULL	effectiveness 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies in our laboratory demonstrating the effectiveness of rovIL-1 as an adjuvant in single and multi-component bacterial toxoid vaccines , and studies from other laboratories demonstrating the application of rbovIL-1 as an adjuvant for the response in cattle to live attenuated viral vaccines , suggest that rIL-1 may become the adjuvant of choice for diseases where protection is mediated by high levels of circulating antibody ( Ab ) .
	manualset3
129807	4	405997	13	NULL	NULL	0	NULL	rovIL-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies in our laboratory demonstrating the effectiveness of rovIL-1 as an adjuvant in single and multi-component bacterial toxoid vaccines , and studies from other laboratories demonstrating the application of rbovIL-1 as an adjuvant for the response in cattle to live attenuated viral vaccines , suggest that rIL-1 may become the adjuvant of choice for diseases where protection is mediated by high levels of circulating antibody ( Ab ) .
	manualset3
129808	5	405997	13	NULL	NULL	0	NULL	adjuvant	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies in our laboratory demonstrating the effectiveness of rovIL-1 as an adjuvant in single and multi-component bacterial toxoid vaccines , and studies from other laboratories demonstrating the application of rbovIL-1 as an adjuvant for the response in cattle to live attenuated viral vaccines , suggest that rIL-1 may become the adjuvant of choice for diseases where protection is mediated by high levels of circulating antibody ( Ab ) .
	manualset3
129809	6	405997	13	NULL	NULL	0	NULL	single bacterial toxoid vaccines	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies in our laboratory demonstrating the effectiveness of rovIL-1 as an adjuvant in single and multi-component bacterial toxoid vaccines , and studies from other laboratories demonstrating the application of rbovIL-1 as an adjuvant for the response in cattle to live attenuated viral vaccines , suggest that rIL-1 may become the adjuvant of choice for diseases where protection is mediated by high levels of circulating antibody ( Ab ) .
	manualset3
129810	7	405997	13	NULL	NULL	0	NULL	multi-component bacterial toxoid vaccines	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies in our laboratory demonstrating the effectiveness of rovIL-1 as an adjuvant in single and multi-component bacterial toxoid vaccines , and studies from other laboratories demonstrating the application of rbovIL-1 as an adjuvant for the response in cattle to live attenuated viral vaccines , suggest that rIL-1 may become the adjuvant of choice for diseases where protection is mediated by high levels of circulating antibody ( Ab ) .
	manualset3
129811	8	405997	13	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies in our laboratory demonstrating the effectiveness of rovIL-1 as an adjuvant in single and multi-component bacterial toxoid vaccines , and studies from other laboratories demonstrating the application of rbovIL-1 as an adjuvant for the response in cattle to live attenuated viral vaccines , suggest that rIL-1 may become the adjuvant of choice for diseases where protection is mediated by high levels of circulating antibody ( Ab ) .
	manualset3
129812	9	405997	13	NULL	NULL	0	NULL	laboratories 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies in our laboratory demonstrating the effectiveness of rovIL-1 as an adjuvant in single and multi-component bacterial toxoid vaccines , and studies from other laboratories demonstrating the application of rbovIL-1 as an adjuvant for the response in cattle to live attenuated viral vaccines , suggest that rIL-1 may become the adjuvant of choice for diseases where protection is mediated by high levels of circulating antibody ( Ab ) .
	manualset3
129813	10	405997	13	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies in our laboratory demonstrating the effectiveness of rovIL-1 as an adjuvant in single and multi-component bacterial toxoid vaccines , and studies from other laboratories demonstrating the application of rbovIL-1 as an adjuvant for the response in cattle to live attenuated viral vaccines , suggest that rIL-1 may become the adjuvant of choice for diseases where protection is mediated by high levels of circulating antibody ( Ab ) .
	manualset3
129814	11	405997	13	NULL	NULL	0	NULL	rbovIL-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies in our laboratory demonstrating the effectiveness of rovIL-1 as an adjuvant in single and multi-component bacterial toxoid vaccines , and studies from other laboratories demonstrating the application of rbovIL-1 as an adjuvant for the response in cattle to live attenuated viral vaccines , suggest that rIL-1 may become the adjuvant of choice for diseases where protection is mediated by high levels of circulating antibody ( Ab ) .
	manualset3
129815	12	405997	13	NULL	NULL	0	NULL	adjuvant	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies in our laboratory demonstrating the effectiveness of rovIL-1 as an adjuvant in single and multi-component bacterial toxoid vaccines , and studies from other laboratories demonstrating the application of rbovIL-1 as an adjuvant for the response in cattle to live attenuated viral vaccines , suggest that rIL-1 may become the adjuvant of choice for diseases where protection is mediated by high levels of circulating antibody ( Ab ) .
	manualset3
129816	13	405997	13	NULL	NULL	0	NULL	response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies in our laboratory demonstrating the effectiveness of rovIL-1 as an adjuvant in single and multi-component bacterial toxoid vaccines , and studies from other laboratories demonstrating the application of rbovIL-1 as an adjuvant for the response in cattle to live attenuated viral vaccines , suggest that rIL-1 may become the adjuvant of choice for diseases where protection is mediated by high levels of circulating antibody ( Ab ) .
	manualset3
129817	14	405997	13	NULL	NULL	0	NULL	cattle	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies in our laboratory demonstrating the effectiveness of rovIL-1 as an adjuvant in single and multi-component bacterial toxoid vaccines , and studies from other laboratories demonstrating the application of rbovIL-1 as an adjuvant for the response in cattle to live attenuated viral vaccines , suggest that rIL-1 may become the adjuvant of choice for diseases where protection is mediated by high levels of circulating antibody ( Ab ) .
	manualset3
129818	15	405997	13	NULL	NULL	0	NULL	viral vaccines 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies in our laboratory demonstrating the effectiveness of rovIL-1 as an adjuvant in single and multi-component bacterial toxoid vaccines , and studies from other laboratories demonstrating the application of rbovIL-1 as an adjuvant for the response in cattle to live attenuated viral vaccines , suggest that rIL-1 may become the adjuvant of choice for diseases where protection is mediated by high levels of circulating antibody ( Ab ) .
	manualset3
129819	16	405997	13	NULL	NULL	NULL	NULL	rIL-1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Recent studies in our laboratory demonstrating the effectiveness of rovIL-1 as an adjuvant in single and multi-component bacterial toxoid vaccines , and studies from other laboratories demonstrating the application of rbovIL-1 as an adjuvant for the response in cattle to live attenuated viral vaccines , suggest that rIL-1 may become the adjuvant of choice for diseases where protection is mediated by high levels of circulating antibody ( Ab ) .
	manualset3
129820	17	405997	13	NULL	NULL	0	NULL	 adjuvant	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies in our laboratory demonstrating the effectiveness of rovIL-1 as an adjuvant in single and multi-component bacterial toxoid vaccines , and studies from other laboratories demonstrating the application of rbovIL-1 as an adjuvant for the response in cattle to live attenuated viral vaccines , suggest that rIL-1 may become the adjuvant of choice for diseases where protection is mediated by high levels of circulating antibody ( Ab ) .
	manualset3
129821	18	405997	13	NULL	NULL	0	NULL	choice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies in our laboratory demonstrating the effectiveness of rovIL-1 as an adjuvant in single and multi-component bacterial toxoid vaccines , and studies from other laboratories demonstrating the application of rbovIL-1 as an adjuvant for the response in cattle to live attenuated viral vaccines , suggest that rIL-1 may become the adjuvant of choice for diseases where protection is mediated by high levels of circulating antibody ( Ab ) .
	manualset3
129822	19	405997	13	NULL	NULL	0	NULL	diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies in our laboratory demonstrating the effectiveness of rovIL-1 as an adjuvant in single and multi-component bacterial toxoid vaccines , and studies from other laboratories demonstrating the application of rbovIL-1 as an adjuvant for the response in cattle to live attenuated viral vaccines , suggest that rIL-1 may become the adjuvant of choice for diseases where protection is mediated by high levels of circulating antibody ( Ab ) .
	manualset3
129823	20	405997	13	NULL	NULL	0	NULL	protection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies in our laboratory demonstrating the effectiveness of rovIL-1 as an adjuvant in single and multi-component bacterial toxoid vaccines , and studies from other laboratories demonstrating the application of rbovIL-1 as an adjuvant for the response in cattle to live attenuated viral vaccines , suggest that rIL-1 may become the adjuvant of choice for diseases where protection is mediated by high levels of circulating antibody ( Ab ) .
	manualset3
129824	21	405997	13	NULL	NULL	0	NULL	high levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies in our laboratory demonstrating the effectiveness of rovIL-1 as an adjuvant in single and multi-component bacterial toxoid vaccines , and studies from other laboratories demonstrating the application of rbovIL-1 as an adjuvant for the response in cattle to live attenuated viral vaccines , suggest that rIL-1 may become the adjuvant of choice for diseases where protection is mediated by high levels of circulating antibody ( Ab ) .
	manualset3
129825	22	405997	13	NULL	NULL	0	NULL	circulating antibody ( Ab )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies in our laboratory demonstrating the effectiveness of rovIL-1 as an adjuvant in single and multi-component bacterial toxoid vaccines , and studies from other laboratories demonstrating the application of rbovIL-1 as an adjuvant for the response in cattle to live attenuated viral vaccines , suggest that rIL-1 may become the adjuvant of choice for diseases where protection is mediated by high levels of circulating antibody ( Ab ) .
	manualset3
129826	1	405998	13	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies indicate that sexual transmission of human immunodeficiency virus type 1 ( HIV-1 ) generally results from productive infection by only one virus , a finding attributable to the mucosal barrier .
	manualset3
129827	2	405998	13	NULL	NULL	0	NULL	sexual transmission	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies indicate that sexual transmission of human immunodeficiency virus type 1 ( HIV-1 ) generally results from productive infection by only one virus , a finding attributable to the mucosal barrier .
	manualset3
129828	3	405998	13	NULL	NULL	0	NULL	human immunodeficiency virus type 1 ( HIV-1 )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies indicate that sexual transmission of human immunodeficiency virus type 1 ( HIV-1 ) generally results from productive infection by only one virus , a finding attributable to the mucosal barrier .
	manualset3
129829	4	405998	13	NULL	NULL	0	NULL	infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies indicate that sexual transmission of human immunodeficiency virus type 1 ( HIV-1 ) generally results from productive infection by only one virus , a finding attributable to the mucosal barrier .
	manualset3
129830	5	405998	13	NULL	NULL	0	NULL	one virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies indicate that sexual transmission of human immunodeficiency virus type 1 ( HIV-1 ) generally results from productive infection by only one virus , a finding attributable to the mucosal barrier .
	manualset3
129831	6	405998	13	NULL	NULL	0	NULL	mucosal barrier	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies indicate that sexual transmission of human immunodeficiency virus type 1 ( HIV-1 ) generally results from productive infection by only one virus , a finding attributable to the mucosal barrier .
	manualset3
129832	1	405999	13	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies of the epidermis in patients with recessive X-linked ichthyosis indicate that cholesterol sulfate is an important endogenous substrate for steroid sulfatase in the stratum corneum .
	manualset3
129833	2	405999	13	NULL	NULL	0	NULL	epidermis	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies of the epidermis in patients with recessive X-linked ichthyosis indicate that cholesterol sulfate is an important endogenous substrate for steroid sulfatase in the stratum corneum .
	manualset3
129834	3	405999	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies of the epidermis in patients with recessive X-linked ichthyosis indicate that cholesterol sulfate is an important endogenous substrate for steroid sulfatase in the stratum corneum .
	manualset3
129835	4	405999	13	NULL	NULL	0	NULL	recessive X-linked ichthyosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies of the epidermis in patients with recessive X-linked ichthyosis indicate that cholesterol sulfate is an important endogenous substrate for steroid sulfatase in the stratum corneum .
	manualset3
129836	5	405999	13	NULL	NULL	0	NULL	cholesterol sulfate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies of the epidermis in patients with recessive X-linked ichthyosis indicate that cholesterol sulfate is an important endogenous substrate for steroid sulfatase in the stratum corneum .
	manualset3
129837	6	405999	13	NULL	NULL	0	NULL	endogenous substrate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies of the epidermis in patients with recessive X-linked ichthyosis indicate that cholesterol sulfate is an important endogenous substrate for steroid sulfatase in the stratum corneum .
	manualset3
129838	7	405999	13	NULL	NULL	0	NULL	 steroid sulfatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies of the epidermis in patients with recessive X-linked ichthyosis indicate that cholesterol sulfate is an important endogenous substrate for steroid sulfatase in the stratum corneum .
	manualset3
129839	8	405999	13	NULL	NULL	0	NULL	stratum corneum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies of the epidermis in patients with recessive X-linked ichthyosis indicate that cholesterol sulfate is an important endogenous substrate for steroid sulfatase in the stratum corneum .
	manualset3
129840	1	406000	13	NULL	NULL	0	NULL	millimolar K ( i )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A millimolar K ( i ) for a statin drug confirmed that E. faecalis HMG-CoA reductase is a class II enzyme .
	manualset3
129841	2	406000	13	NULL	NULL	0	NULL	statin drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A millimolar K ( i ) for a statin drug confirmed that E. faecalis HMG-CoA reductase is a class II enzyme .
	manualset3
129842	3	406000	13	NULL	NULL	0	NULL	E. faecalis HMG-CoA reductase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A millimolar K ( i ) for a statin drug confirmed that E. faecalis HMG-CoA reductase is a class II enzyme .
	manualset3
129843	4	406000	13	NULL	NULL	0	NULL	class II enzyme 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A millimolar K ( i ) for a statin drug confirmed that E. faecalis HMG-CoA reductase is a class II enzyme .
	manualset3
129844	1	406001	13	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies suggest that this may increase mortality in patients with hypovolaemic shock .
	manualset3
129845	2	406001	13	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies suggest that this may increase mortality in patients with hypovolaemic shock .
	manualset3
129846	3	406001	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies suggest that this may increase mortality in patients with hypovolaemic shock .
	manualset3
129847	4	406001	13	NULL	NULL	0	NULL	hypovolaemic shock	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies suggest that this may increase mortality in patients with hypovolaemic shock .
	manualset3
129848	1	406002	13	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies using mutant mice have expanded our knowledge of the key roles that abnormalities in synaptic function and formation play in epileptogenesis , and further illustrate just how closely some mouse models resemble human epilepsy .
	manualset3
129849	2	406002	13	NULL	NULL	0	NULL	mutant mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies using mutant mice have expanded our knowledge of the key roles that abnormalities in synaptic function and formation play in epileptogenesis , and further illustrate just how closely some mouse models resemble human epilepsy .
	manualset3
129850	3	406002	13	NULL	NULL	0	NULL	knowledge	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies using mutant mice have expanded our knowledge of the key roles that abnormalities in synaptic function and formation play in epileptogenesis , and further illustrate just how closely some mouse models resemble human epilepsy .
	manualset3
129851	4	406002	13	NULL	NULL	0	NULL	key roles	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies using mutant mice have expanded our knowledge of the key roles that abnormalities in synaptic function and formation play in epileptogenesis , and further illustrate just how closely some mouse models resemble human epilepsy .
	manualset3
129852	5	406002	13	NULL	NULL	0	NULL	abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies using mutant mice have expanded our knowledge of the key roles that abnormalities in synaptic function and formation play in epileptogenesis , and further illustrate just how closely some mouse models resemble human epilepsy .
	manualset3
129853	6	406002	13	NULL	NULL	0	NULL	synaptic function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies using mutant mice have expanded our knowledge of the key roles that abnormalities in synaptic function and formation play in epileptogenesis , and further illustrate just how closely some mouse models resemble human epilepsy .
	manualset3
129854	7	406002	13	NULL	NULL	0	NULL	formation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies using mutant mice have expanded our knowledge of the key roles that abnormalities in synaptic function and formation play in epileptogenesis , and further illustrate just how closely some mouse models resemble human epilepsy .
	manualset3
129855	8	406002	13	NULL	NULL	0	NULL	epileptogenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies using mutant mice have expanded our knowledge of the key roles that abnormalities in synaptic function and formation play in epileptogenesis , and further illustrate just how closely some mouse models resemble human epilepsy .
	manualset3
129856	9	406002	13	NULL	NULL	0	NULL	mouse models 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies using mutant mice have expanded our knowledge of the key roles that abnormalities in synaptic function and formation play in epileptogenesis , and further illustrate just how closely some mouse models resemble human epilepsy .
	manualset3
129857	10	406002	13	NULL	NULL	0	NULL	human epilepsy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies using mutant mice have expanded our knowledge of the key roles that abnormalities in synaptic function and formation play in epileptogenesis , and further illustrate just how closely some mouse models resemble human epilepsy .
	manualset3
129858	1	406003	13	NULL	NULL	0	NULL	technological progress 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent technological progress has increased the number of techniques available for blood purification and their performance .
	manualset3
129859	2	406003	13	NULL	NULL	0	NULL	number of techniques	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent technological progress has increased the number of techniques available for blood purification and their performance .
	manualset3
129860	3	406003	13	NULL	NULL	0	NULL	blood purification	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent technological progress has increased the number of techniques available for blood purification and their performance .
	manualset3
129861	4	406003	13	NULL	NULL	0	NULL	performance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent technological progress has increased the number of techniques available for blood purification and their performance .
	manualset3
129862	1	406004	13	NULL	NULL	0	NULL	trends 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent trends in macro - , micro - , and nanomaterial-based tools and strategies for heavy-metal detection .
	manualset3
129863	2	406004	13	NULL	NULL	0	NULL	macro -based tools 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent trends in macro - , micro - , and nanomaterial-based tools and strategies for heavy-metal detection .
	manualset3
129864	3	406004	13	NULL	NULL	0	NULL	micro -based tools	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent trends in macro - , micro - , and nanomaterial-based tools and strategies for heavy-metal detection .
	manualset3
129865	4	406004	13	NULL	NULL	0	NULL	nanomaterial-based tools 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent trends in macro - , micro - , and nanomaterial-based tools and strategies for heavy-metal detection .
	manualset3
129866	5	406004	13	NULL	NULL	0	NULL	strategies	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent trends in macro - , micro - , and nanomaterial-based tools and strategies for heavy-metal detection .
	manualset3
129867	6	406004	13	NULL	NULL	0	NULL	heavy-metal detection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent trends in macro - , micro - , and nanomaterial-based tools and strategies for heavy-metal detection .
	manualset3
129868	1	406005	13	NULL	NULL	NULL	NULL	work	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Recent work has also involved using the model to study the alloreactivity of cord blood .
	manualset3
129869	2	406005	13	NULL	NULL	0	NULL	model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent work has also involved using the model to study the alloreactivity of cord blood .
	manualset3
129870	3	406005	13	NULL	NULL	0	NULL	alloreactivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent work has also involved using the model to study the alloreactivity of cord blood .
	manualset3
129871	4	406005	13	NULL	NULL	0	NULL	cord blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent work has also involved using the model to study the alloreactivity of cord blood .
	manualset3
129872	1	406006	13	NULL	NULL	0	NULL	work	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent work with plants has demonstrated that genome instability can be triggered by a change in chromosome number arising from either whole genome duplications ( polyploidy ) or loss/gain of individual chromosomes ( aneuploidy ) .
	manualset3
129873	2	406006	13	NULL	NULL	0	NULL	plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent work with plants has demonstrated that genome instability can be triggered by a change in chromosome number arising from either whole genome duplications ( polyploidy ) or loss/gain of individual chromosomes ( aneuploidy ) .
	manualset3
129874	3	406006	13	NULL	NULL	0	NULL	genome instability 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent work with plants has demonstrated that genome instability can be triggered by a change in chromosome number arising from either whole genome duplications ( polyploidy ) or loss/gain of individual chromosomes ( aneuploidy ) .
	manualset3
129875	4	406006	13	NULL	NULL	0	NULL	change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent work with plants has demonstrated that genome instability can be triggered by a change in chromosome number arising from either whole genome duplications ( polyploidy ) or loss/gain of individual chromosomes ( aneuploidy ) .
	manualset3
129876	5	406006	13	NULL	NULL	0	NULL	chromosome number	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent work with plants has demonstrated that genome instability can be triggered by a change in chromosome number arising from either whole genome duplications ( polyploidy ) or loss/gain of individual chromosomes ( aneuploidy ) .
	manualset3
129877	6	406006	13	NULL	NULL	0	NULL	genome duplications ( polyploidy )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent work with plants has demonstrated that genome instability can be triggered by a change in chromosome number arising from either whole genome duplications ( polyploidy ) or loss/gain of individual chromosomes ( aneuploidy ) .
	manualset3
129878	7	406006	13	NULL	NULL	0	NULL	loss/gain of individual chromosomes ( aneuploidy )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent work with plants has demonstrated that genome instability can be triggered by a change in chromosome number arising from either whole genome duplications ( polyploidy ) or loss/gain of individual chromosomes ( aneuploidy ) .
	manualset3
129879	1	406007	13	NULL	NULL	0	NULL	2 randomized trials	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , 2 randomized trials , comparing definitive chemoradiation with chemoradiation and surgery were published .
	manualset3
129880	2	406007	13	NULL	NULL	0	NULL	chemoradiation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , 2 randomized trials , comparing definitive chemoradiation with chemoradiation and surgery were published .
	manualset3
129881	3	406007	13	NULL	NULL	0	NULL	chemoradiation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , 2 randomized trials , comparing definitive chemoradiation with chemoradiation and surgery were published .
	manualset3
129882	4	406007	13	NULL	NULL	0	NULL	surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , 2 randomized trials , comparing definitive chemoradiation with chemoradiation and surgery were published .
	manualset3
129883	1	406008	13	NULL	NULL	0	NULL	COL2A1 mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , COL2A1 mutations were shown to be associated with milder forms of chondrodysplasia , which may present with precocious generalized osteoarthritis ( OA ) .
	manualset3
129884	2	406008	13	NULL	NULL	0	NULL	milder forms of chondrodysplasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , COL2A1 mutations were shown to be associated with milder forms of chondrodysplasia , which may present with precocious generalized osteoarthritis ( OA ) .
	manualset3
129885	3	406008	13	NULL	NULL	0	NULL	osteoarthritis ( OA )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , COL2A1 mutations were shown to be associated with milder forms of chondrodysplasia , which may present with precocious generalized osteoarthritis ( OA ) .
	manualset3
129886	1	406009	13	NULL	NULL	0	NULL	DNA restriction endonuclease analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , DNA restriction endonuclease analysis has been used for typing of P. gingivalis , Pr .
	manualset3
129887	2	406009	13	NULL	NULL	0	NULL	typing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , DNA restriction endonuclease analysis has been used for typing of P. gingivalis , Pr .
	manualset3
129888	3	406009	13	NULL	NULL	0	NULL	P. gingivalis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , DNA restriction endonuclease analysis has been used for typing of P. gingivalis , Pr .
	manualset3
129889	1	406010	13	NULL	NULL	0	NULL	DNR 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , DNR has been replaced in many centers by idarubicin ( IDA ) as the first choice anthracycline in AML treatment .
	manualset3
129890	2	406010	13	NULL	NULL	0	NULL	centers	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , DNR has been replaced in many centers by idarubicin ( IDA ) as the first choice anthracycline in AML treatment .
	manualset3
129891	3	406010	13	NULL	NULL	0	NULL	idarubicin ( IDA ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , DNR has been replaced in many centers by idarubicin ( IDA ) as the first choice anthracycline in AML treatment .
	manualset3
129892	4	406010	13	NULL	NULL	NULL	NULL	choice 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Recently , DNR has been replaced in many centers by idarubicin ( IDA ) as the first choice anthracycline in AML treatment .
	manualset3
129893	5	406010	13	NULL	NULL	0	NULL	anthracycline	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , DNR has been replaced in many centers by idarubicin ( IDA ) as the first choice anthracycline in AML treatment .
	manualset3
129894	6	406010	13	NULL	NULL	0	NULL	AML treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , DNR has been replaced in many centers by idarubicin ( IDA ) as the first choice anthracycline in AML treatment .
	manualset3
129895	1	406011	13	NULL	NULL	0	NULL	NEIL1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , NEIL1 , a human homolog of Escherichia coli DNA glycosylase endonuclease VIII , has been identified and shown to exhibit broad substrate specificity for a variety of types of pyrimidine-base damage .
	manualset3
129896	2	406011	13	NULL	NULL	0	NULL	 human homolog of Escherichia coli DNA glycosylase endonuclease VIII	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , NEIL1 , a human homolog of Escherichia coli DNA glycosylase endonuclease VIII , has been identified and shown to exhibit broad substrate specificity for a variety of types of pyrimidine-base damage .
	manualset3
129897	3	406011	13	NULL	NULL	0	NULL	substrate specificity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , NEIL1 , a human homolog of Escherichia coli DNA glycosylase endonuclease VIII , has been identified and shown to exhibit broad substrate specificity for a variety of types of pyrimidine-base damage .
	manualset3
129898	4	406011	13	NULL	NULL	0	NULL	variety of types 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , NEIL1 , a human homolog of Escherichia coli DNA glycosylase endonuclease VIII , has been identified and shown to exhibit broad substrate specificity for a variety of types of pyrimidine-base damage .
	manualset3
129899	5	406011	13	NULL	NULL	0	NULL	pyrimidine-base damage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , NEIL1 , a human homolog of Escherichia coli DNA glycosylase endonuclease VIII , has been identified and shown to exhibit broad substrate specificity for a variety of types of pyrimidine-base damage .
	manualset3
129900	1	406012	13	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , a new protein in the neutrophil granules , human neutrophil lipocalin ( HNL ) has been discovered .
	manualset3
129901	2	406012	13	NULL	NULL	0	NULL	neutrophil granules	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , a new protein in the neutrophil granules , human neutrophil lipocalin ( HNL ) has been discovered .
	manualset3
129902	3	406012	13	NULL	NULL	0	NULL	human neutrophil lipocalin ( HNL )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , a new protein in the neutrophil granules , human neutrophil lipocalin ( HNL ) has been discovered .
	manualset3
129903	1	406013	13	NULL	NULL	0	NULL	novel function 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , a novel function of Twist1 was reported to confer radioresistance or chemoresistance in cervical cancer .
	manualset3
129904	2	406013	13	NULL	NULL	0	NULL	Twist1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , a novel function of Twist1 was reported to confer radioresistance or chemoresistance in cervical cancer .
	manualset3
129905	3	406013	13	NULL	NULL	0	NULL	radioresistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , a novel function of Twist1 was reported to confer radioresistance or chemoresistance in cervical cancer .
	manualset3
129906	4	406013	13	NULL	NULL	0	NULL	chemoresistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , a novel function of Twist1 was reported to confer radioresistance or chemoresistance in cervical cancer .
	manualset3
129907	5	406013	13	NULL	NULL	0	NULL	cervical cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , a novel function of Twist1 was reported to confer radioresistance or chemoresistance in cervical cancer .
	manualset3
129908	1	406014	13	NULL	NULL	0	NULL	number	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , a number of circulating apoptosis biomarkers have emerged , such as full-length and caspase-cleaved cytokeratin 18 ( CK18 ) and nucleosomal DNA ( nDNA ) , that may be predictive of likely outcome .
	manualset3
129909	2	406014	13	NULL	NULL	0	NULL	circulating apoptosis biomarkers 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , a number of circulating apoptosis biomarkers have emerged , such as full-length and caspase-cleaved cytokeratin 18 ( CK18 ) and nucleosomal DNA ( nDNA ) , that may be predictive of likely outcome .
	manualset3
129910	3	406014	13	NULL	NULL	0	NULL	full-length cytokeratin 18 ( CK18 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , a number of circulating apoptosis biomarkers have emerged , such as full-length and caspase-cleaved cytokeratin 18 ( CK18 ) and nucleosomal DNA ( nDNA ) , that may be predictive of likely outcome .
	manualset3
129911	4	406014	13	NULL	NULL	0	NULL	caspase-cleaved cytokeratin 18 ( CK18 )	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , a number of circulating apoptosis biomarkers have emerged , such as full-length and caspase-cleaved cytokeratin 18 ( CK18 ) and nucleosomal DNA ( nDNA ) , that may be predictive of likely outcome .
	manualset3
129912	5	406014	13	NULL	NULL	0	NULL	nucleosomal DNA ( nDNA ) 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , a number of circulating apoptosis biomarkers have emerged , such as full-length and caspase-cleaved cytokeratin 18 ( CK18 ) and nucleosomal DNA ( nDNA ) , that may be predictive of likely outcome .
	manualset3
129913	6	406014	13	NULL	NULL	0	NULL	outcome	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , a number of circulating apoptosis biomarkers have emerged , such as full-length and caspase-cleaved cytokeratin 18 ( CK18 ) and nucleosomal DNA ( nDNA ) , that may be predictive of likely outcome .
	manualset3
129914	1	406015	13	NULL	NULL	0	NULL	drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , an interesting drug represented by ezetimibe has been found that may provide cholesterol-lowering additive to that reached with statin treatment .
	manualset3
129915	2	406015	13	NULL	NULL	0	NULL	ezetimibe	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , an interesting drug represented by ezetimibe has been found that may provide cholesterol-lowering additive to that reached with statin treatment .
	manualset3
129916	3	406015	13	NULL	NULL	0	NULL	cholesterol-lowering additive	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , an interesting drug represented by ezetimibe has been found that may provide cholesterol-lowering additive to that reached with statin treatment .
	manualset3
129917	4	406015	13	NULL	NULL	0	NULL	statin treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , an interesting drug represented by ezetimibe has been found that may provide cholesterol-lowering additive to that reached with statin treatment .
	manualset3
129918	1	406016	13	NULL	NULL	0	NULL	five SRIF receptor subtypes ( SSTR1-5 )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , five SRIF receptor subtypes ( SSTR1-5 ) have been cloned , all of which bind SRIF with high affinity .
	manualset3
129919	2	406016	13	NULL	NULL	0	NULL	bind	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , five SRIF receptor subtypes ( SSTR1-5 ) have been cloned , all of which bind SRIF with high affinity .
	manualset3
129920	3	406016	13	NULL	NULL	0	NULL	SRIF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , five SRIF receptor subtypes ( SSTR1-5 ) have been cloned , all of which bind SRIF with high affinity .
	manualset3
129921	4	406016	13	NULL	NULL	0	NULL	high affinity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , five SRIF receptor subtypes ( SSTR1-5 ) have been cloned , all of which bind SRIF with high affinity .
	manualset3
129922	1	406017	13	NULL	NULL	0	NULL	interest 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , however , interest in these signals was spurred as they were proposed as potential control signals for neuronal motor prostheses , i.e. , for devices fit to record and decode brain activity to restore motor functions in paralyzed patients .
	manualset3
129923	2	406017	13	NULL	NULL	0	NULL	signals 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , however , interest in these signals was spurred as they were proposed as potential control signals for neuronal motor prostheses , i.e. , for devices fit to record and decode brain activity to restore motor functions in paralyzed patients .
	manualset3
129924	3	406017	13	NULL	NULL	0	NULL	control signals	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , however , interest in these signals was spurred as they were proposed as potential control signals for neuronal motor prostheses , i.e. , for devices fit to record and decode brain activity to restore motor functions in paralyzed patients .
	manualset3
129925	4	406017	13	NULL	NULL	0	NULL	neuronal motor prostheses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , however , interest in these signals was spurred as they were proposed as potential control signals for neuronal motor prostheses , i.e. , for devices fit to record and decode brain activity to restore motor functions in paralyzed patients .
	manualset3
129926	5	406017	13	NULL	NULL	0	NULL	devices	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , however , interest in these signals was spurred as they were proposed as potential control signals for neuronal motor prostheses , i.e. , for devices fit to record and decode brain activity to restore motor functions in paralyzed patients .
	manualset3
129927	6	406017	13	NULL	NULL	0	NULL	brain activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , however , interest in these signals was spurred as they were proposed as potential control signals for neuronal motor prostheses , i.e. , for devices fit to record and decode brain activity to restore motor functions in paralyzed patients .
	manualset3
129928	7	406017	13	NULL	NULL	0	NULL	motor functions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , however , interest in these signals was spurred as they were proposed as potential control signals for neuronal motor prostheses , i.e. , for devices fit to record and decode brain activity to restore motor functions in paralyzed patients .
	manualset3
129929	8	406017	13	NULL	NULL	0	NULL	paralyzed patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , however , interest in these signals was spurred as they were proposed as potential control signals for neuronal motor prostheses , i.e. , for devices fit to record and decode brain activity to restore motor functions in paralyzed patients .
	manualset3
129930	1	406018	13	NULL	NULL	0	NULL	RAG proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , it has been shown that RAG proteins thus induced are functional and can mediate the secondary rearrangement of Ig genes ( receptor editing ) at mature stages of B cells .
	manualset3
129931	2	406018	13	NULL	NULL	0	NULL	secondary rearrangement	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , it has been shown that RAG proteins thus induced are functional and can mediate the secondary rearrangement of Ig genes ( receptor editing ) at mature stages of B cells .
	manualset3
129932	3	406018	13	NULL	NULL	0	NULL	Ig genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , it has been shown that RAG proteins thus induced are functional and can mediate the secondary rearrangement of Ig genes ( receptor editing ) at mature stages of B cells .
	manualset3
129933	4	406018	13	NULL	NULL	0	NULL	receptor editing 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , it has been shown that RAG proteins thus induced are functional and can mediate the secondary rearrangement of Ig genes ( receptor editing ) at mature stages of B cells .
	manualset3
129934	5	406018	13	NULL	NULL	0	NULL	mature stages	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , it has been shown that RAG proteins thus induced are functional and can mediate the secondary rearrangement of Ig genes ( receptor editing ) at mature stages of B cells .
	manualset3
129935	6	406018	13	NULL	NULL	0	NULL	B cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , it has been shown that RAG proteins thus induced are functional and can mediate the secondary rearrangement of Ig genes ( receptor editing ) at mature stages of B cells .
	manualset3
129936	1	406019	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	( -3 t ) ; the data strongly suggest that this isomer is the 1-propene-1-thiol radical cation , namely CH3CH = CH-SH + . .
	manualset3
129937	2	406019	13	NULL	NULL	NULL	NULL	isomer	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( -3 t ) ; the data strongly suggest that this isomer is the 1-propene-1-thiol radical cation , namely CH3CH = CH-SH + . .
	manualset3
129938	3	406019	13	NULL	NULL	0	NULL	1-propene-1-thiol radical cation 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	( -3 t ) ; the data strongly suggest that this isomer is the 1-propene-1-thiol radical cation , namely CH3CH = CH-SH + . .
	manualset3
129939	4	406019	13	NULL	NULL	0	NULL	CH3CH = CH-SH +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	( -3 t ) ; the data strongly suggest that this isomer is the 1-propene-1-thiol radical cation , namely CH3CH = CH-SH + . .
	manualset3
129940	1	406020	13	NULL	NULL	0	NULL	Clinical evaluation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3 ) Clinical evaluation of ivabradine only includes randomised controlled trials versus two other anti-angina drugs : atenolol and amlodipine .
	manualset3
129941	2	406020	13	NULL	NULL	0	NULL	ivabradine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3 ) Clinical evaluation of ivabradine only includes randomised controlled trials versus two other anti-angina drugs : atenolol and amlodipine .
	manualset3
129942	3	406020	13	NULL	NULL	0	NULL	 randomised controlled trials	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3 ) Clinical evaluation of ivabradine only includes randomised controlled trials versus two other anti-angina drugs : atenolol and amlodipine .
	manualset3
129943	4	406020	13	NULL	NULL	0	NULL	two other anti-angina drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3 ) Clinical evaluation of ivabradine only includes randomised controlled trials versus two other anti-angina drugs : atenolol and amlodipine .
	manualset3
129944	5	406020	13	NULL	NULL	0	NULL	atenolol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3 ) Clinical evaluation of ivabradine only includes randomised controlled trials versus two other anti-angina drugs : atenolol and amlodipine .
	manualset3
129945	6	406020	13	NULL	NULL	0	NULL	amlodipine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3 ) Clinical evaluation of ivabradine only includes randomised controlled trials versus two other anti-angina drugs : atenolol and amlodipine .
	manualset3
129946	1	406021	13	NULL	NULL	0	NULL	Capillary sprouting 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Capillary sprouting as a reparation principle in local radiation injuries ) .
	manualset3
129947	2	406021	13	NULL	NULL	0	NULL	reparation principle	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Capillary sprouting as a reparation principle in local radiation injuries ) .
	manualset3
129948	3	406021	13	NULL	NULL	0	NULL	local radiation injuries	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Capillary sprouting as a reparation principle in local radiation injuries ) .
	manualset3
129949	1	406022	13	NULL	NULL	0	NULL	minigenerator	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A minigenerator for the production of krypton-81m and its applications .
	manualset3
129950	2	406022	13	NULL	NULL	0	NULL	production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A minigenerator for the production of krypton-81m and its applications .
	manualset3
129951	3	406022	13	NULL	NULL	0	NULL	krypton-81m	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	A minigenerator for the production of krypton-81m and its applications .
	manualset3
129952	4	406022	13	NULL	NULL	0	NULL	applications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A minigenerator for the production of krypton-81m and its applications .
	manualset3
129953	1	406023	13	NULL	NULL	0	NULL	constitutionality 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , its constitutionality was challenged on the basis of 1 ) the vagueness of statutory aims to pursue public health versus the individual privacy interests of cancer patients , and 2 ) the alleged indignity of one 's individual medical information being transmitted to government authorities .
	manualset3
129954	2	406023	13	NULL	NULL	0	NULL	basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , its constitutionality was challenged on the basis of 1 ) the vagueness of statutory aims to pursue public health versus the individual privacy interests of cancer patients , and 2 ) the alleged indignity of one 's individual medical information being transmitted to government authorities .
	manualset3
129955	3	406023	13	NULL	NULL	0	NULL	vagueness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , its constitutionality was challenged on the basis of 1 ) the vagueness of statutory aims to pursue public health versus the individual privacy interests of cancer patients , and 2 ) the alleged indignity of one 's individual medical information being transmitted to government authorities .
	manualset3
129956	4	406023	13	NULL	NULL	0	NULL	statutory aims	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , its constitutionality was challenged on the basis of 1 ) the vagueness of statutory aims to pursue public health versus the individual privacy interests of cancer patients , and 2 ) the alleged indignity of one 's individual medical information being transmitted to government authorities .
	manualset3
129957	5	406023	13	NULL	NULL	0	NULL	public health 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , its constitutionality was challenged on the basis of 1 ) the vagueness of statutory aims to pursue public health versus the individual privacy interests of cancer patients , and 2 ) the alleged indignity of one 's individual medical information being transmitted to government authorities .
	manualset3
129958	6	406023	13	NULL	NULL	0	NULL	 individual privacy interests 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , its constitutionality was challenged on the basis of 1 ) the vagueness of statutory aims to pursue public health versus the individual privacy interests of cancer patients , and 2 ) the alleged indignity of one 's individual medical information being transmitted to government authorities .
	manualset3
129959	7	406023	13	NULL	NULL	0	NULL	cancer patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , its constitutionality was challenged on the basis of 1 ) the vagueness of statutory aims to pursue public health versus the individual privacy interests of cancer patients , and 2 ) the alleged indignity of one 's individual medical information being transmitted to government authorities .
	manualset3
129960	8	406023	13	NULL	NULL	0	NULL	indignity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , its constitutionality was challenged on the basis of 1 ) the vagueness of statutory aims to pursue public health versus the individual privacy interests of cancer patients , and 2 ) the alleged indignity of one 's individual medical information being transmitted to government authorities .
	manualset3
129961	9	406023	13	NULL	NULL	0	NULL	medical information	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , its constitutionality was challenged on the basis of 1 ) the vagueness of statutory aims to pursue public health versus the individual privacy interests of cancer patients , and 2 ) the alleged indignity of one 's individual medical information being transmitted to government authorities .
	manualset3
129962	10	406023	13	NULL	NULL	0	NULL	government authorities 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , its constitutionality was challenged on the basis of 1 ) the vagueness of statutory aims to pursue public health versus the individual privacy interests of cancer patients , and 2 ) the alleged indignity of one 's individual medical information being transmitted to government authorities .
	manualset3
129963	1	406024	13	NULL	NULL	0	NULL	radiologists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , radiologists have formed collaborations with molecular biologists and chemists in order to develop molecular agents that target cancer cells via receptor-substrate or specific physiochemical interactions .
	manualset3
129964	2	406024	13	NULL	NULL	0	NULL	collaborations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , radiologists have formed collaborations with molecular biologists and chemists in order to develop molecular agents that target cancer cells via receptor-substrate or specific physiochemical interactions .
	manualset3
129965	3	406024	13	NULL	NULL	0	NULL	molecular biologists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , radiologists have formed collaborations with molecular biologists and chemists in order to develop molecular agents that target cancer cells via receptor-substrate or specific physiochemical interactions .
	manualset3
129966	4	406024	13	NULL	NULL	0	NULL	chemists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , radiologists have formed collaborations with molecular biologists and chemists in order to develop molecular agents that target cancer cells via receptor-substrate or specific physiochemical interactions .
	manualset3
129968	6	406024	13	NULL	NULL	0	NULL	molecular agents	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , radiologists have formed collaborations with molecular biologists and chemists in order to develop molecular agents that target cancer cells via receptor-substrate or specific physiochemical interactions .
	manualset3
129970	8	406024	13	NULL	NULL	0	NULL	cancer cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , radiologists have formed collaborations with molecular biologists and chemists in order to develop molecular agents that target cancer cells via receptor-substrate or specific physiochemical interactions .
	manualset3
129971	9	406024	13	NULL	NULL	0	NULL	receptor-substrate interactions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , radiologists have formed collaborations with molecular biologists and chemists in order to develop molecular agents that target cancer cells via receptor-substrate or specific physiochemical interactions .
	manualset3
129972	10	406024	13	NULL	NULL	0	NULL	specific physiochemical interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , radiologists have formed collaborations with molecular biologists and chemists in order to develop molecular agents that target cancer cells via receptor-substrate or specific physiochemical interactions .
	manualset3
129973	1	406025	13	NULL	NULL	0	NULL	reports	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , several reports have revealed the importance of SUMO in the function of a variety of repressor complexes .
	manualset3
129974	2	406025	13	NULL	NULL	0	NULL	importance	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , several reports have revealed the importance of SUMO in the function of a variety of repressor complexes .
	manualset3
129975	3	406025	13	NULL	NULL	0	NULL	SUMO	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , several reports have revealed the importance of SUMO in the function of a variety of repressor complexes .
	manualset3
129976	4	406025	13	NULL	NULL	0	NULL	function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , several reports have revealed the importance of SUMO in the function of a variety of repressor complexes .
	manualset3
129977	5	406025	13	NULL	NULL	0	NULL	variety of repressor complexes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , several reports have revealed the importance of SUMO in the function of a variety of repressor complexes .
	manualset3
129978	1	406026	13	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , the authors reported that the concurrent knockdown of PKC and , via upregulating PKC , sensitizes cells with aberrant Ras signaling to apoptosis .
	manualset3
129979	2	406026	13	NULL	NULL	0	NULL	concurrent knockdown	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , the authors reported that the concurrent knockdown of PKC and , via upregulating PKC , sensitizes cells with aberrant Ras signaling to apoptosis .
	manualset3
129980	3	406026	13	NULL	NULL	0	NULL	PKC	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , the authors reported that the concurrent knockdown of PKC and , via upregulating PKC , sensitizes cells with aberrant Ras signaling to apoptosis .
	manualset3
129981	4	406026	13	NULL	NULL	NULL	NULL	PKC	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Recently , the authors reported that the concurrent knockdown of PKC and , via upregulating PKC , sensitizes cells with aberrant Ras signaling to apoptosis .
	manualset3
129982	5	406026	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , the authors reported that the concurrent knockdown of PKC and , via upregulating PKC , sensitizes cells with aberrant Ras signaling to apoptosis .
	manualset3
129983	6	406026	13	NULL	NULL	0	NULL	Ras signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , the authors reported that the concurrent knockdown of PKC and , via upregulating PKC , sensitizes cells with aberrant Ras signaling to apoptosis .
	manualset3
129984	7	406026	13	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , the authors reported that the concurrent knockdown of PKC and , via upregulating PKC , sensitizes cells with aberrant Ras signaling to apoptosis .
	manualset3
129985	1	406027	13	NULL	NULL	0	NULL	power of epidemiology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , the power of epidemiology as a primary investigative tool has grown to the point where unsuspected associations between occupation and cancer risk may be the first hint that a problem exists .
	manualset3
129986	2	406027	13	NULL	NULL	0	NULL	primary investigative tool 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , the power of epidemiology as a primary investigative tool has grown to the point where unsuspected associations between occupation and cancer risk may be the first hint that a problem exists .
	manualset3
129987	3	406027	13	NULL	NULL	0	NULL	associations 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , the power of epidemiology as a primary investigative tool has grown to the point where unsuspected associations between occupation and cancer risk may be the first hint that a problem exists .
	manualset3
129988	4	406027	13	NULL	NULL	0	NULL	occupation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , the power of epidemiology as a primary investigative tool has grown to the point where unsuspected associations between occupation and cancer risk may be the first hint that a problem exists .
	manualset3
129989	5	406027	13	NULL	NULL	0	NULL	cancer risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , the power of epidemiology as a primary investigative tool has grown to the point where unsuspected associations between occupation and cancer risk may be the first hint that a problem exists .
	manualset3
129990	6	406027	13	NULL	NULL	0	NULL	hint	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , the power of epidemiology as a primary investigative tool has grown to the point where unsuspected associations between occupation and cancer risk may be the first hint that a problem exists .
	manualset3
129991	7	406027	13	NULL	NULL	0	NULL	problem	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , the power of epidemiology as a primary investigative tool has grown to the point where unsuspected associations between occupation and cancer risk may be the first hint that a problem exists .
	manualset3
129992	1	406028	13	NULL	NULL	0	NULL	three-dimensional structure 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , the three-dimensional structure of the active site of human DNA polymerase alpha ( pol alpha ) was proposed based on the application of molecular modeling methods and molecular dynamic simulations .
	manualset3
129993	2	406028	13	NULL	NULL	0	NULL	active site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , the three-dimensional structure of the active site of human DNA polymerase alpha ( pol alpha ) was proposed based on the application of molecular modeling methods and molecular dynamic simulations .
	manualset3
129994	3	406028	13	NULL	NULL	0	NULL	human DNA polymerase alpha ( pol alpha )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , the three-dimensional structure of the active site of human DNA polymerase alpha ( pol alpha ) was proposed based on the application of molecular modeling methods and molecular dynamic simulations .
	manualset3
129995	4	406028	13	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , the three-dimensional structure of the active site of human DNA polymerase alpha ( pol alpha ) was proposed based on the application of molecular modeling methods and molecular dynamic simulations .
	manualset3
129996	5	406028	13	NULL	NULL	0	NULL	molecular modeling methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , the three-dimensional structure of the active site of human DNA polymerase alpha ( pol alpha ) was proposed based on the application of molecular modeling methods and molecular dynamic simulations .
	manualset3
129997	6	406028	13	NULL	NULL	0	NULL	molecular dynamic simulations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , the three-dimensional structure of the active site of human DNA polymerase alpha ( pol alpha ) was proposed based on the application of molecular modeling methods and molecular dynamic simulations .
	manualset3
129998	1	406029	13	NULL	NULL	0	NULL	models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we derived models for predicting intestinal permeability using the hydrogen bonding descriptors polar surface area ( PSA ) and number of hydrogen bond donors ( HBD ) , and a lipophilicity descriptor ( J. Med .
	manualset3
129999	2	406029	13	NULL	NULL	0	NULL	intestinal permeability 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we derived models for predicting intestinal permeability using the hydrogen bonding descriptors polar surface area ( PSA ) and number of hydrogen bond donors ( HBD ) , and a lipophilicity descriptor ( J. Med .
	manualset3
130000	3	406029	13	NULL	NULL	0	NULL	 hydrogen bonding descriptors polar surface area ( PSA ) 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we derived models for predicting intestinal permeability using the hydrogen bonding descriptors polar surface area ( PSA ) and number of hydrogen bond donors ( HBD ) , and a lipophilicity descriptor ( J. Med .
	manualset3
130001	4	406029	13	NULL	NULL	0	NULL	hydrogen bond donors ( HBD )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we derived models for predicting intestinal permeability using the hydrogen bonding descriptors polar surface area ( PSA ) and number of hydrogen bond donors ( HBD ) , and a lipophilicity descriptor ( J. Med .
	manualset3
130002	5	406029	13	NULL	NULL	0	NULL	lipophilicity descriptor 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we derived models for predicting intestinal permeability using the hydrogen bonding descriptors polar surface area ( PSA ) and number of hydrogen bond donors ( HBD ) , and a lipophilicity descriptor ( J. Med .
	manualset3
130003	6	406029	13	NULL	NULL	0	NULL	J. Med 	Journal												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we derived models for predicting intestinal permeability using the hydrogen bonding descriptors polar surface area ( PSA ) and number of hydrogen bond donors ( HBD ) , and a lipophilicity descriptor ( J. Med .
	manualset3
130004	1	406030	13	NULL	NULL	0	NULL	functional recognition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we found that the specific functional recognition of apoptotic cells is a ubiquitous property of virtually all cell types , including mouse embryo fibroblasts , and reflects an innate immunity that discriminates live from effete cells .
	manualset3
130005	2	406030	13	NULL	NULL	0	NULL	apoptotic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we found that the specific functional recognition of apoptotic cells is a ubiquitous property of virtually all cell types , including mouse embryo fibroblasts , and reflects an innate immunity that discriminates live from effete cells .
	manualset3
130006	3	406030	13	NULL	NULL	0	NULL	ubiquitous property 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we found that the specific functional recognition of apoptotic cells is a ubiquitous property of virtually all cell types , including mouse embryo fibroblasts , and reflects an innate immunity that discriminates live from effete cells .
	manualset3
130007	4	406030	13	NULL	NULL	0	NULL	cell types	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we found that the specific functional recognition of apoptotic cells is a ubiquitous property of virtually all cell types , including mouse embryo fibroblasts , and reflects an innate immunity that discriminates live from effete cells .
	manualset3
130008	5	406030	13	NULL	NULL	0	NULL	mouse embryo fibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we found that the specific functional recognition of apoptotic cells is a ubiquitous property of virtually all cell types , including mouse embryo fibroblasts , and reflects an innate immunity that discriminates live from effete cells .
	manualset3
130009	6	406030	13	NULL	NULL	0	NULL	innate immunity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we found that the specific functional recognition of apoptotic cells is a ubiquitous property of virtually all cell types , including mouse embryo fibroblasts , and reflects an innate immunity that discriminates live from effete cells .
	manualset3
130010	7	406030	13	NULL	NULL	0	NULL	effete cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we found that the specific functional recognition of apoptotic cells is a ubiquitous property of virtually all cell types , including mouse embryo fibroblasts , and reflects an innate immunity that discriminates live from effete cells .
	manualset3
130011	8	406030	13	NULL	NULL	0	NULL	live cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we found that the specific functional recognition of apoptotic cells is a ubiquitous property of virtually all cell types , including mouse embryo fibroblasts , and reflects an innate immunity that discriminates live from effete cells .
	manualset3
130450	1	406031	13	NULL	NULL	NULL	NULL	minor population of donors	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A minor population of donors with a high rate of energy transfer can produce sensitized acceptor decay which is dominated by a decay component corresponding to this minor donor population .
	manualset3
130451	2	406031	13	NULL	NULL	0	NULL	rate of energy transfer	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A minor population of donors with a high rate of energy transfer can produce sensitized acceptor decay which is dominated by a decay component corresponding to this minor donor population .
	manualset3
130452	3	406031	13	NULL	NULL	0	NULL	acceptor decay	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A minor population of donors with a high rate of energy transfer can produce sensitized acceptor decay which is dominated by a decay component corresponding to this minor donor population .
	manualset3
130453	4	406031	13	NULL	NULL	0	NULL	decay component 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A minor population of donors with a high rate of energy transfer can produce sensitized acceptor decay which is dominated by a decay component corresponding to this minor donor population .
	manualset3
130454	5	406031	13	NULL	NULL	0	NULL	minor donor population	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A minor population of donors with a high rate of energy transfer can produce sensitized acceptor decay which is dominated by a decay component corresponding to this minor donor population .
	manualset3
130455	1	406032	13	NULL	NULL	0	NULL	database	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we reported a database ( Noncoded Amino acids Database ; http : //recerca.upc.edu/imem/index.htm ) that was built to compile information about the intrinsic conformational preferences of nonproteinogenic residues determined by quantum mechanical calculations , as well as bibliographic information about their synthesis , physical and spectroscopic characterization , the experimentally established conformational propensities , and applications ( Revilla-Lpez et al. , J Phys Chem B 2010 ; 114 : 7413 -7422 ) .
	manualset3
130456	2	406032	13	NULL	NULL	0	NULL	Amino acids Database	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we reported a database ( Noncoded Amino acids Database ; http : //recerca.upc.edu/imem/index.htm ) that was built to compile information about the intrinsic conformational preferences of nonproteinogenic residues determined by quantum mechanical calculations , as well as bibliographic information about their synthesis , physical and spectroscopic characterization , the experimentally established conformational propensities , and applications ( Revilla-Lpez et al. , J Phys Chem B 2010 ; 114 : 7413 -7422 ) .
	manualset3
130457	3	406032	13	NULL	NULL	0	NULL	information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we reported a database ( Noncoded Amino acids Database ; http : //recerca.upc.edu/imem/index.htm ) that was built to compile information about the intrinsic conformational preferences of nonproteinogenic residues determined by quantum mechanical calculations , as well as bibliographic information about their synthesis , physical and spectroscopic characterization , the experimentally established conformational propensities , and applications ( Revilla-Lpez et al. , J Phys Chem B 2010 ; 114 : 7413 -7422 ) .
	manualset3
130458	4	406032	13	NULL	NULL	0	NULL	conformational preferences	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we reported a database ( Noncoded Amino acids Database ; http : //recerca.upc.edu/imem/index.htm ) that was built to compile information about the intrinsic conformational preferences of nonproteinogenic residues determined by quantum mechanical calculations , as well as bibliographic information about their synthesis , physical and spectroscopic characterization , the experimentally established conformational propensities , and applications ( Revilla-Lpez et al. , J Phys Chem B 2010 ; 114 : 7413 -7422 ) .
	manualset3
130459	5	406032	13	NULL	NULL	0	NULL	nonproteinogenic residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we reported a database ( Noncoded Amino acids Database ; http : //recerca.upc.edu/imem/index.htm ) that was built to compile information about the intrinsic conformational preferences of nonproteinogenic residues determined by quantum mechanical calculations , as well as bibliographic information about their synthesis , physical and spectroscopic characterization , the experimentally established conformational propensities , and applications ( Revilla-Lpez et al. , J Phys Chem B 2010 ; 114 : 7413 -7422 ) .
	manualset3
130460	6	406032	13	NULL	NULL	0	NULL	quantum mechanical calculations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we reported a database ( Noncoded Amino acids Database ; http : //recerca.upc.edu/imem/index.htm ) that was built to compile information about the intrinsic conformational preferences of nonproteinogenic residues determined by quantum mechanical calculations , as well as bibliographic information about their synthesis , physical and spectroscopic characterization , the experimentally established conformational propensities , and applications ( Revilla-Lpez et al. , J Phys Chem B 2010 ; 114 : 7413 -7422 ) .
	manualset3
130461	7	406032	13	NULL	NULL	0	NULL	bibliographic information 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we reported a database ( Noncoded Amino acids Database ; http : //recerca.upc.edu/imem/index.htm ) that was built to compile information about the intrinsic conformational preferences of nonproteinogenic residues determined by quantum mechanical calculations , as well as bibliographic information about their synthesis , physical and spectroscopic characterization , the experimentally established conformational propensities , and applications ( Revilla-Lpez et al. , J Phys Chem B 2010 ; 114 : 7413 -7422 ) .
	manualset3
130462	8	406032	13	NULL	NULL	0	NULL	synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we reported a database ( Noncoded Amino acids Database ; http : //recerca.upc.edu/imem/index.htm ) that was built to compile information about the intrinsic conformational preferences of nonproteinogenic residues determined by quantum mechanical calculations , as well as bibliographic information about their synthesis , physical and spectroscopic characterization , the experimentally established conformational propensities , and applications ( Revilla-Lpez et al. , J Phys Chem B 2010 ; 114 : 7413 -7422 ) .
	manualset3
130463	9	406032	13	NULL	NULL	0	NULL	physical characterization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we reported a database ( Noncoded Amino acids Database ; http : //recerca.upc.edu/imem/index.htm ) that was built to compile information about the intrinsic conformational preferences of nonproteinogenic residues determined by quantum mechanical calculations , as well as bibliographic information about their synthesis , physical and spectroscopic characterization , the experimentally established conformational propensities , and applications ( Revilla-Lpez et al. , J Phys Chem B 2010 ; 114 : 7413 -7422 ) .
	manualset3
130464	10	406032	13	NULL	NULL	0	NULL	spectroscopic characterization 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we reported a database ( Noncoded Amino acids Database ; http : //recerca.upc.edu/imem/index.htm ) that was built to compile information about the intrinsic conformational preferences of nonproteinogenic residues determined by quantum mechanical calculations , as well as bibliographic information about their synthesis , physical and spectroscopic characterization , the experimentally established conformational propensities , and applications ( Revilla-Lpez et al. , J Phys Chem B 2010 ; 114 : 7413 -7422 ) .
	manualset3
130465	11	406032	13	NULL	NULL	0	NULL	conformational propensities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we reported a database ( Noncoded Amino acids Database ; http : //recerca.upc.edu/imem/index.htm ) that was built to compile information about the intrinsic conformational preferences of nonproteinogenic residues determined by quantum mechanical calculations , as well as bibliographic information about their synthesis , physical and spectroscopic characterization , the experimentally established conformational propensities , and applications ( Revilla-Lpez et al. , J Phys Chem B 2010 ; 114 : 7413 -7422 ) .
	manualset3
130466	12	406032	13	NULL	NULL	0	NULL	applications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we reported a database ( Noncoded Amino acids Database ; http : //recerca.upc.edu/imem/index.htm ) that was built to compile information about the intrinsic conformational preferences of nonproteinogenic residues determined by quantum mechanical calculations , as well as bibliographic information about their synthesis , physical and spectroscopic characterization , the experimentally established conformational propensities , and applications ( Revilla-Lpez et al. , J Phys Chem B 2010 ; 114 : 7413 -7422 ) .
	manualset3
130467	13	406032	13	NULL	NULL	0	NULL	Revilla-Lpez et al	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we reported a database ( Noncoded Amino acids Database ; http : //recerca.upc.edu/imem/index.htm ) that was built to compile information about the intrinsic conformational preferences of nonproteinogenic residues determined by quantum mechanical calculations , as well as bibliographic information about their synthesis , physical and spectroscopic characterization , the experimentally established conformational propensities , and applications ( Revilla-Lpez et al. , J Phys Chem B 2010 ; 114 : 7413 -7422 ) .
	manualset3
130468	14	406032	13	NULL	NULL	0	NULL	J Phys Chem B 2010 	Journal												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we reported a database ( Noncoded Amino acids Database ; http : //recerca.upc.edu/imem/index.htm ) that was built to compile information about the intrinsic conformational preferences of nonproteinogenic residues determined by quantum mechanical calculations , as well as bibliographic information about their synthesis , physical and spectroscopic characterization , the experimentally established conformational propensities , and applications ( Revilla-Lpez et al. , J Phys Chem B 2010 ; 114 : 7413 -7422 ) .
	manualset3
130469	1	406033	13	NULL	NULL	0	NULL	levels 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently high levels of protection against tomato spotted wilt virus ( TSWV ) , a negative-strand RNA virus infecting plants , have been obtained by transforming tobacco with viral nucleoprotein ( N ) gene sequences .
	manualset3
130470	2	406033	13	NULL	NULL	0	NULL	protection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently high levels of protection against tomato spotted wilt virus ( TSWV ) , a negative-strand RNA virus infecting plants , have been obtained by transforming tobacco with viral nucleoprotein ( N ) gene sequences .
	manualset3
130471	3	406033	13	NULL	NULL	0	NULL	tomato spotted wilt virus ( TSWV ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently high levels of protection against tomato spotted wilt virus ( TSWV ) , a negative-strand RNA virus infecting plants , have been obtained by transforming tobacco with viral nucleoprotein ( N ) gene sequences .
	manualset3
130472	4	406033	13	NULL	NULL	0	NULL	negative-strand RNA virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently high levels of protection against tomato spotted wilt virus ( TSWV ) , a negative-strand RNA virus infecting plants , have been obtained by transforming tobacco with viral nucleoprotein ( N ) gene sequences .
	manualset3
130473	5	406033	13	NULL	NULL	0	NULL	plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently high levels of protection against tomato spotted wilt virus ( TSWV ) , a negative-strand RNA virus infecting plants , have been obtained by transforming tobacco with viral nucleoprotein ( N ) gene sequences .
	manualset3
130474	6	406033	13	NULL	NULL	0	NULL	tobacco 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently high levels of protection against tomato spotted wilt virus ( TSWV ) , a negative-strand RNA virus infecting plants , have been obtained by transforming tobacco with viral nucleoprotein ( N ) gene sequences .
	manualset3
130475	7	406033	13	NULL	NULL	0	NULL	viral nucleoprotein ( N ) gene sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently high levels of protection against tomato spotted wilt virus ( TSWV ) , a negative-strand RNA virus infecting plants , have been obtained by transforming tobacco with viral nucleoprotein ( N ) gene sequences .
	manualset3
130476	1	406034	13	NULL	NULL	0	NULL	glass vessels	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently marketed glass vessels that are uniform and pass USP specifications were compared with uniform plastic vessels that also pass USP specifications .
	manualset3
130477	2	406034	13	NULL	NULL	0	NULL	USP specifications 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently marketed glass vessels that are uniform and pass USP specifications were compared with uniform plastic vessels that also pass USP specifications .
	manualset3
130478	3	406034	13	NULL	NULL	0	NULL	uniform plastic vessels	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently marketed glass vessels that are uniform and pass USP specifications were compared with uniform plastic vessels that also pass USP specifications .
	manualset3
130479	4	406034	13	NULL	NULL	0	NULL	USP specifications 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently marketed glass vessels that are uniform and pass USP specifications were compared with uniform plastic vessels that also pass USP specifications .
	manualset3
130480	1	406035	13	NULL	NULL	0	NULL	Receptor-activated release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Receptor-activated release of taurine from glia represents a previously undescribed neuronal-glial interaction by which glia may actively regulate neuronal excitability .
	manualset3
130481	2	406035	13	NULL	NULL	0	NULL	taurine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Receptor-activated release of taurine from glia represents a previously undescribed neuronal-glial interaction by which glia may actively regulate neuronal excitability .
	manualset3
130482	3	406035	13	NULL	NULL	0	NULL	glia	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Receptor-activated release of taurine from glia represents a previously undescribed neuronal-glial interaction by which glia may actively regulate neuronal excitability .
	manualset3
130483	4	406035	13	NULL	NULL	0	NULL	neuronal-glial interaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Receptor-activated release of taurine from glia represents a previously undescribed neuronal-glial interaction by which glia may actively regulate neuronal excitability .
	manualset3
130484	5	406035	13	NULL	NULL	0	NULL	glia 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Receptor-activated release of taurine from glia represents a previously undescribed neuronal-glial interaction by which glia may actively regulate neuronal excitability .
	manualset3
130485	6	406035	13	NULL	NULL	0	NULL	neuronal excitability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Receptor-activated release of taurine from glia represents a previously undescribed neuronal-glial interaction by which glia may actively regulate neuronal excitability .
	manualset3
130486	1	406036	13	NULL	NULL	0	NULL	Receptor occupancy	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Receptor occupancy was measured using the antagonist ( 3H ) prazosin and correlated with agonist-elicited 45Ca2 + fluxes .
	manualset3
130487	2	406036	13	NULL	NULL	0	NULL	antagonist ( 3H ) prazosin 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Receptor occupancy was measured using the antagonist ( 3H ) prazosin and correlated with agonist-elicited 45Ca2 + fluxes .
	manualset3
130488	3	406036	13	NULL	NULL	0	NULL	45Ca2 + fluxes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Receptor occupancy was measured using the antagonist ( 3H ) prazosin and correlated with agonist-elicited 45Ca2 + fluxes .
	manualset3
130489	1	406037	13	NULL	NULL	0	NULL	epigenetic modification 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reciprocal epigenetic modification of histone H2B occurs in chromatin during apoptosis in vitro and in vivo .
	manualset3
130490	2	406037	13	NULL	NULL	0	NULL	histone H2B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Reciprocal epigenetic modification of histone H2B occurs in chromatin during apoptosis in vitro and in vivo .
	manualset3
130491	3	406037	13	NULL	NULL	0	NULL	chromatin	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Reciprocal epigenetic modification of histone H2B occurs in chromatin during apoptosis in vitro and in vivo .
	manualset3
130492	4	406037	13	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reciprocal epigenetic modification of histone H2B occurs in chromatin during apoptosis in vitro and in vivo .
	manualset3
130493	1	406038	13	NULL	NULL	0	NULL	Reciprocal relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Reciprocal relationships between insulin resistance and endothelial dysfunction : molecular and pathophysiological mechanisms .
	manualset3
130494	2	406038	13	NULL	NULL	0	NULL	insulin resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reciprocal relationships between insulin resistance and endothelial dysfunction : molecular and pathophysiological mechanisms .
	manualset3
130495	3	406038	13	NULL	NULL	0	NULL	endothelial dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reciprocal relationships between insulin resistance and endothelial dysfunction : molecular and pathophysiological mechanisms .
	manualset3
130496	4	406038	13	NULL	NULL	0	NULL	molecular mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reciprocal relationships between insulin resistance and endothelial dysfunction : molecular and pathophysiological mechanisms .
	manualset3
130497	5	406038	13	NULL	NULL	0	NULL	pathophysiological mechanisms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reciprocal relationships between insulin resistance and endothelial dysfunction : molecular and pathophysiological mechanisms .
	manualset3
130498	1	406039	13	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reciprocally , reduction of Cdk1 activity by knockdown of mitotic cyclins extended pre-MBT S phase .
	manualset3
130499	2	406039	13	NULL	NULL	0	NULL	Cdk1 activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reciprocally , reduction of Cdk1 activity by knockdown of mitotic cyclins extended pre-MBT S phase .
	manualset3
130500	3	406039	13	NULL	NULL	0	NULL	knockdown	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Reciprocally , reduction of Cdk1 activity by knockdown of mitotic cyclins extended pre-MBT S phase .
	manualset3
130501	4	406039	13	NULL	NULL	0	NULL	mitotic cyclins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Reciprocally , reduction of Cdk1 activity by knockdown of mitotic cyclins extended pre-MBT S phase .
	manualset3
130502	5	406039	13	NULL	NULL	0	NULL	pre-MBT S phase	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Reciprocally , reduction of Cdk1 activity by knockdown of mitotic cyclins extended pre-MBT S phase .
	manualset3
130503	1	406040	13	NULL	NULL	0	NULL	interdependence	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognising the clear interdependence between the right to food and the right to health , this paper explores how international human rights obligations could inform approaches to addressing food poverty and insecurity with specific reference to Ireland and the UK .
	manualset3
130504	2	406040	13	NULL	NULL	NULL	NULL	right to food 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Recognising the clear interdependence between the right to food and the right to health , this paper explores how international human rights obligations could inform approaches to addressing food poverty and insecurity with specific reference to Ireland and the UK .
	manualset3
130505	3	406040	13	NULL	NULL	0	NULL	right to health	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognising the clear interdependence between the right to food and the right to health , this paper explores how international human rights obligations could inform approaches to addressing food poverty and insecurity with specific reference to Ireland and the UK .
	manualset3
130506	4	406040	13	NULL	NULL	0	NULL	paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognising the clear interdependence between the right to food and the right to health , this paper explores how international human rights obligations could inform approaches to addressing food poverty and insecurity with specific reference to Ireland and the UK .
	manualset3
130507	5	406040	13	NULL	NULL	0	NULL	international human rights obligations	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognising the clear interdependence between the right to food and the right to health , this paper explores how international human rights obligations could inform approaches to addressing food poverty and insecurity with specific reference to Ireland and the UK .
	manualset3
130508	6	406040	13	NULL	NULL	0	NULL	approaches	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognising the clear interdependence between the right to food and the right to health , this paper explores how international human rights obligations could inform approaches to addressing food poverty and insecurity with specific reference to Ireland and the UK .
	manualset3
130509	7	406040	13	NULL	NULL	0	NULL	food poverty	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognising the clear interdependence between the right to food and the right to health , this paper explores how international human rights obligations could inform approaches to addressing food poverty and insecurity with specific reference to Ireland and the UK .
	manualset3
130510	8	406040	13	NULL	NULL	0	NULL	insecurity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognising the clear interdependence between the right to food and the right to health , this paper explores how international human rights obligations could inform approaches to addressing food poverty and insecurity with specific reference to Ireland and the UK .
	manualset3
130511	9	406040	13	NULL	NULL	0	NULL	reference 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognising the clear interdependence between the right to food and the right to health , this paper explores how international human rights obligations could inform approaches to addressing food poverty and insecurity with specific reference to Ireland and the UK .
	manualset3
130512	10	406040	13	NULL	NULL	0	NULL	Ireland	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognising the clear interdependence between the right to food and the right to health , this paper explores how international human rights obligations could inform approaches to addressing food poverty and insecurity with specific reference to Ireland and the UK .
	manualset3
130513	11	406040	13	NULL	NULL	0	NULL	UK	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognising the clear interdependence between the right to food and the right to health , this paper explores how international human rights obligations could inform approaches to addressing food poverty and insecurity with specific reference to Ireland and the UK .
	manualset3
130514	1	406041	13	NULL	NULL	0	NULL	mixture	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A mixture of methylene and azure blue was used for specimen7 .
	manualset3
130515	2	406041	13	NULL	NULL	0	NULL	methylene 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A mixture of methylene and azure blue was used for specimen7 .
	manualset3
130516	3	406041	13	NULL	NULL	0	NULL	azure blue	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A mixture of methylene and azure blue was used for specimen7 .
	manualset3
130517	4	406041	13	NULL	NULL	0	NULL	specimen7 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A mixture of methylene and azure blue was used for specimen7 .
	manualset3
130518	1	406042	13	NULL	NULL	0	NULL	Recognition events	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition events in AM symbiosis : analysis of fungal gene expression at the early appressorium stage .
	manualset3
130519	2	406042	13	NULL	NULL	0	NULL	AM symbiosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition events in AM symbiosis : analysis of fungal gene expression at the early appressorium stage .
	manualset3
130520	3	406042	13	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition events in AM symbiosis : analysis of fungal gene expression at the early appressorium stage .
	manualset3
130521	4	406042	13	NULL	NULL	0	NULL	fungal gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition events in AM symbiosis : analysis of fungal gene expression at the early appressorium stage .
	manualset3
130522	5	406042	13	NULL	NULL	0	NULL	early appressorium stage	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition events in AM symbiosis : analysis of fungal gene expression at the early appressorium stage .
	manualset3
130523	1	406043	13	NULL	NULL	0	NULL	Recognition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of cisplatin-DNA interstrand cross-links by replication protein A .
	manualset3
130524	2	406043	13	NULL	NULL	0	NULL	cisplatin-DNA interstrand cross-links 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of cisplatin-DNA interstrand cross-links by replication protein A .
	manualset3
130525	3	406043	13	NULL	NULL	0	NULL	replication protein A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of cisplatin-DNA interstrand cross-links by replication protein A .
	manualset3
130526	1	406044	13	NULL	NULL	0	NULL	Recognition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of the association between a hand condition and ocular pathology may aid in diagnosis of a systemic disorder or allow early detection and prevention of ocular disease and loss of vision .
	manualset3
130527	2	406044	13	NULL	NULL	0	NULL	association 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of the association between a hand condition and ocular pathology may aid in diagnosis of a systemic disorder or allow early detection and prevention of ocular disease and loss of vision .
	manualset3
130528	3	406044	13	NULL	NULL	0	NULL	hand condition 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of the association between a hand condition and ocular pathology may aid in diagnosis of a systemic disorder or allow early detection and prevention of ocular disease and loss of vision .
	manualset3
130529	4	406044	13	NULL	NULL	0	NULL	ocular pathology 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of the association between a hand condition and ocular pathology may aid in diagnosis of a systemic disorder or allow early detection and prevention of ocular disease and loss of vision .
	manualset3
130530	5	406044	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of the association between a hand condition and ocular pathology may aid in diagnosis of a systemic disorder or allow early detection and prevention of ocular disease and loss of vision .
	manualset3
130531	6	406044	13	NULL	NULL	0	NULL	systemic disorder	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of the association between a hand condition and ocular pathology may aid in diagnosis of a systemic disorder or allow early detection and prevention of ocular disease and loss of vision .
	manualset3
130532	7	406044	13	NULL	NULL	0	NULL	detection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of the association between a hand condition and ocular pathology may aid in diagnosis of a systemic disorder or allow early detection and prevention of ocular disease and loss of vision .
	manualset3
130533	8	406044	13	NULL	NULL	0	NULL	prevention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of the association between a hand condition and ocular pathology may aid in diagnosis of a systemic disorder or allow early detection and prevention of ocular disease and loss of vision .
	manualset3
130534	9	406044	13	NULL	NULL	0	NULL	ocular disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of the association between a hand condition and ocular pathology may aid in diagnosis of a systemic disorder or allow early detection and prevention of ocular disease and loss of vision .
	manualset3
130535	10	406044	13	NULL	NULL	0	NULL	loss of vision 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of the association between a hand condition and ocular pathology may aid in diagnosis of a systemic disorder or allow early detection and prevention of ocular disease and loss of vision .
	manualset3
130536	1	406045	13	NULL	NULL	0	NULL	Recognition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of the possibility of vocal cord paralysis in an abused child who suffers significant head trauma or a strangulation injury is necessary to insure a more rapid diagnosis and initiation of effective therapy more promptly .
	manualset3
130537	2	406045	13	NULL	NULL	0	NULL	possibility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of the possibility of vocal cord paralysis in an abused child who suffers significant head trauma or a strangulation injury is necessary to insure a more rapid diagnosis and initiation of effective therapy more promptly .
	manualset3
130538	3	406045	13	NULL	NULL	0	NULL	vocal cord paralysis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of the possibility of vocal cord paralysis in an abused child who suffers significant head trauma or a strangulation injury is necessary to insure a more rapid diagnosis and initiation of effective therapy more promptly .
	manualset3
130539	4	406045	13	NULL	NULL	0	NULL	child	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of the possibility of vocal cord paralysis in an abused child who suffers significant head trauma or a strangulation injury is necessary to insure a more rapid diagnosis and initiation of effective therapy more promptly .
	manualset3
130540	5	406045	13	NULL	NULL	0	NULL	 head trauma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of the possibility of vocal cord paralysis in an abused child who suffers significant head trauma or a strangulation injury is necessary to insure a more rapid diagnosis and initiation of effective therapy more promptly .
	manualset3
130541	6	406045	13	NULL	NULL	0	NULL	strangulation injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of the possibility of vocal cord paralysis in an abused child who suffers significant head trauma or a strangulation injury is necessary to insure a more rapid diagnosis and initiation of effective therapy more promptly .
	manualset3
130542	7	406045	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of the possibility of vocal cord paralysis in an abused child who suffers significant head trauma or a strangulation injury is necessary to insure a more rapid diagnosis and initiation of effective therapy more promptly .
	manualset3
130543	8	406045	13	NULL	NULL	0	NULL	initiation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of the possibility of vocal cord paralysis in an abused child who suffers significant head trauma or a strangulation injury is necessary to insure a more rapid diagnosis and initiation of effective therapy more promptly .
	manualset3
130544	9	406045	13	NULL	NULL	0	NULL	effective therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of the possibility of vocal cord paralysis in an abused child who suffers significant head trauma or a strangulation injury is necessary to insure a more rapid diagnosis and initiation of effective therapy more promptly .
	manualset3
130545	1	406046	13	NULL	NULL	0	NULL	Recognition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of the significant advantages of minimizing surgical trauma has resulted in a substantial increase in the number of minimally invasive ( MI ) cardiac surgical procedures being performed .
	manualset3
130546	2	406046	13	NULL	NULL	0	NULL	advantages	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of the significant advantages of minimizing surgical trauma has resulted in a substantial increase in the number of minimally invasive ( MI ) cardiac surgical procedures being performed .
	manualset3
130547	3	406046	13	NULL	NULL	0	NULL	surgical trauma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of the significant advantages of minimizing surgical trauma has resulted in a substantial increase in the number of minimally invasive ( MI ) cardiac surgical procedures being performed .
	manualset3
130548	4	406046	13	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of the significant advantages of minimizing surgical trauma has resulted in a substantial increase in the number of minimally invasive ( MI ) cardiac surgical procedures being performed .
	manualset3
130549	5	406046	13	NULL	NULL	0	NULL	number	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of the significant advantages of minimizing surgical trauma has resulted in a substantial increase in the number of minimally invasive ( MI ) cardiac surgical procedures being performed .
	manualset3
130550	6	406046	13	NULL	NULL	0	NULL	minimally invasive ( MI ) cardiac surgical procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of the significant advantages of minimizing surgical trauma has resulted in a substantial increase in the number of minimally invasive ( MI ) cardiac surgical procedures being performed .
	manualset3
130551	1	406047	13	NULL	NULL	0	NULL	Recognition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of these patterns of GI tract involvement by vascular graft infection may facilitate prompt diagnosis and improve treatment results .
	manualset3
130552	2	406047	13	NULL	NULL	0	NULL	patterns	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of these patterns of GI tract involvement by vascular graft infection may facilitate prompt diagnosis and improve treatment results .
	manualset3
130553	3	406047	13	NULL	NULL	0	NULL	GI tract involvement 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of these patterns of GI tract involvement by vascular graft infection may facilitate prompt diagnosis and improve treatment results .
	manualset3
130554	4	406047	13	NULL	NULL	0	NULL	vascular graft infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of these patterns of GI tract involvement by vascular graft infection may facilitate prompt diagnosis and improve treatment results .
	manualset3
130555	5	406047	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of these patterns of GI tract involvement by vascular graft infection may facilitate prompt diagnosis and improve treatment results .
	manualset3
130556	6	406047	13	NULL	NULL	0	NULL	treatment results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognition of these patterns of GI tract involvement by vascular graft infection may facilitate prompt diagnosis and improve treatment results .
	manualset3
130557	1	406048	13	NULL	NULL	0	NULL	Antiquity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognized early in Antiquity by its excessive urine output , its clinical features and fatal outcome were recorded by the end of the first century A.D. by Areteus of Cappadocia and attributed to a weakness of the retentive ability of the kidneys by Galen .
	manualset3
130558	2	406048	13	NULL	NULL	0	NULL	urine output	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognized early in Antiquity by its excessive urine output , its clinical features and fatal outcome were recorded by the end of the first century A.D. by Areteus of Cappadocia and attributed to a weakness of the retentive ability of the kidneys by Galen .
	manualset3
130559	3	406048	13	NULL	NULL	0	NULL	clinical features	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognized early in Antiquity by its excessive urine output , its clinical features and fatal outcome were recorded by the end of the first century A.D. by Areteus of Cappadocia and attributed to a weakness of the retentive ability of the kidneys by Galen .
	manualset3
130560	4	406048	13	NULL	NULL	0	NULL	fatal outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognized early in Antiquity by its excessive urine output , its clinical features and fatal outcome were recorded by the end of the first century A.D. by Areteus of Cappadocia and attributed to a weakness of the retentive ability of the kidneys by Galen .
	manualset3
130561	5	406048	13	NULL	NULL	0	NULL	first century A.D	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognized early in Antiquity by its excessive urine output , its clinical features and fatal outcome were recorded by the end of the first century A.D. by Areteus of Cappadocia and attributed to a weakness of the retentive ability of the kidneys by Galen .
	manualset3
130562	6	406048	13	NULL	NULL	0	NULL	Areteus	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognized early in Antiquity by its excessive urine output , its clinical features and fatal outcome were recorded by the end of the first century A.D. by Areteus of Cappadocia and attributed to a weakness of the retentive ability of the kidneys by Galen .
	manualset3
130563	7	406048	13	NULL	NULL	0	NULL	Cappadocia	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognized early in Antiquity by its excessive urine output , its clinical features and fatal outcome were recorded by the end of the first century A.D. by Areteus of Cappadocia and attributed to a weakness of the retentive ability of the kidneys by Galen .
	manualset3
130564	8	406048	13	NULL	NULL	0	NULL	weakness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognized early in Antiquity by its excessive urine output , its clinical features and fatal outcome were recorded by the end of the first century A.D. by Areteus of Cappadocia and attributed to a weakness of the retentive ability of the kidneys by Galen .
	manualset3
130565	9	406048	13	NULL	NULL	0	NULL	retentive ability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognized early in Antiquity by its excessive urine output , its clinical features and fatal outcome were recorded by the end of the first century A.D. by Areteus of Cappadocia and attributed to a weakness of the retentive ability of the kidneys by Galen .
	manualset3
130566	10	406048	13	NULL	NULL	0	NULL	kidneys	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognized early in Antiquity by its excessive urine output , its clinical features and fatal outcome were recorded by the end of the first century A.D. by Areteus of Cappadocia and attributed to a weakness of the retentive ability of the kidneys by Galen .
	manualset3
130567	11	406048	13	NULL	NULL	0	NULL	Galen	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognized early in Antiquity by its excessive urine output , its clinical features and fatal outcome were recorded by the end of the first century A.D. by Areteus of Cappadocia and attributed to a weakness of the retentive ability of the kidneys by Galen .
	manualset3
130568	12	406048	13	NULL	NULL	0	NULL	end	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognized early in Antiquity by its excessive urine output , its clinical features and fatal outcome were recorded by the end of the first century A.D. by Areteus of Cappadocia and attributed to a weakness of the retentive ability of the kidneys by Galen .
	manualset3
130569	1	406049	13	NULL	NULL	0	NULL	ideal tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognizing the ideal tissue for restoration of function and aesthetics , thin skin dorsally and sensate glabrous skin volarly , is the first step to effective application of microsurgery in the hand .
	manualset3
130570	2	406049	13	NULL	NULL	0	NULL	restoration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognizing the ideal tissue for restoration of function and aesthetics , thin skin dorsally and sensate glabrous skin volarly , is the first step to effective application of microsurgery in the hand .
	manualset3
130571	3	406049	13	NULL	NULL	0	NULL	function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognizing the ideal tissue for restoration of function and aesthetics , thin skin dorsally and sensate glabrous skin volarly , is the first step to effective application of microsurgery in the hand .
	manualset3
130572	4	406049	13	NULL	NULL	0	NULL	aesthetics	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognizing the ideal tissue for restoration of function and aesthetics , thin skin dorsally and sensate glabrous skin volarly , is the first step to effective application of microsurgery in the hand .
	manualset3
130573	5	406049	13	NULL	NULL	0	NULL	skin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognizing the ideal tissue for restoration of function and aesthetics , thin skin dorsally and sensate glabrous skin volarly , is the first step to effective application of microsurgery in the hand .
	manualset3
130574	6	406049	13	NULL	NULL	0	NULL	sensate glabrous skin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognizing the ideal tissue for restoration of function and aesthetics , thin skin dorsally and sensate glabrous skin volarly , is the first step to effective application of microsurgery in the hand .
	manualset3
130575	7	406049	13	NULL	NULL	0	NULL	first step	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognizing the ideal tissue for restoration of function and aesthetics , thin skin dorsally and sensate glabrous skin volarly , is the first step to effective application of microsurgery in the hand .
	manualset3
130576	8	406049	13	NULL	NULL	0	NULL	effective application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognizing the ideal tissue for restoration of function and aesthetics , thin skin dorsally and sensate glabrous skin volarly , is the first step to effective application of microsurgery in the hand .
	manualset3
130577	9	406049	13	NULL	NULL	0	NULL	microsurgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognizing the ideal tissue for restoration of function and aesthetics , thin skin dorsally and sensate glabrous skin volarly , is the first step to effective application of microsurgery in the hand .
	manualset3
130578	10	406049	13	NULL	NULL	0	NULL	hand	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Recognizing the ideal tissue for restoration of function and aesthetics , thin skin dorsally and sensate glabrous skin volarly , is the first step to effective application of microsurgery in the hand .
	manualset3
130579	1	406050	13	NULL	NULL	0	NULL	Recombinant Rho1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant Rho1 confers upon Pkc1 the ability to be stimulated by phosphatidylserine , indicating that Rho1 controls signal transmission through Pkc1 .
	manualset3
130580	2	406050	13	NULL	NULL	0	NULL	Pkc1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant Rho1 confers upon Pkc1 the ability to be stimulated by phosphatidylserine , indicating that Rho1 controls signal transmission through Pkc1 .
	manualset3
130581	3	406050	13	NULL	NULL	0	NULL	ability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant Rho1 confers upon Pkc1 the ability to be stimulated by phosphatidylserine , indicating that Rho1 controls signal transmission through Pkc1 .
	manualset3
130582	4	406050	13	NULL	NULL	0	NULL	phosphatidylserine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant Rho1 confers upon Pkc1 the ability to be stimulated by phosphatidylserine , indicating that Rho1 controls signal transmission through Pkc1 .
	manualset3
130583	5	406050	13	NULL	NULL	0	NULL	Rho1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant Rho1 confers upon Pkc1 the ability to be stimulated by phosphatidylserine , indicating that Rho1 controls signal transmission through Pkc1 .
	manualset3
130584	6	406050	13	NULL	NULL	0	NULL	controls 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant Rho1 confers upon Pkc1 the ability to be stimulated by phosphatidylserine , indicating that Rho1 controls signal transmission through Pkc1 .
	manualset3
130585	7	406050	13	NULL	NULL	0	NULL	signal transmission 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant Rho1 confers upon Pkc1 the ability to be stimulated by phosphatidylserine , indicating that Rho1 controls signal transmission through Pkc1 .
	manualset3
130586	8	406050	13	NULL	NULL	0	NULL	Pkc1	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant Rho1 confers upon Pkc1 the ability to be stimulated by phosphatidylserine , indicating that Rho1 controls signal transmission through Pkc1 .
	manualset3
130587	1	406051	13	NULL	NULL	0	NULL	Recombinant VV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant VV were constructed that constitutively express p67 and inducibly express PKR in BSC-40 cells .
	manualset3
130588	2	406051	13	NULL	NULL	0	NULL	p67 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant VV were constructed that constitutively express p67 and inducibly express PKR in BSC-40 cells .
	manualset3
130589	3	406051	13	NULL	NULL	0	NULL	PKR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant VV were constructed that constitutively express p67 and inducibly express PKR in BSC-40 cells .
	manualset3
130590	4	406051	13	NULL	NULL	0	NULL	BSC-40 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant VV were constructed that constitutively express p67 and inducibly express PKR in BSC-40 cells .
	manualset3
130591	1	406052	13	NULL	NULL	0	NULL	Recombinant endostatin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant endostatin was also purified to homogeneity using a simple one-step Ni2 + affinity fractionation .
	manualset3
130593	2	406052	13	NULL	NULL	0	NULL	homogeneity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant endostatin was also purified to homogeneity using a simple one-step Ni2 + affinity fractionation .
	manualset3
130594	3	406052	13	NULL	NULL	0	NULL	one-step Ni2 + affinity fractionation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant endostatin was also purified to homogeneity using a simple one-step Ni2 + affinity fractionation .
	manualset3
130595	1	406053	13	NULL	NULL	0	NULL	Recombinant factor VIIa	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant factor VIIa reduces transfusion requirements in liver transplant patients with high MELD scores .
	manualset3
130596	2	406053	13	NULL	NULL	0	NULL	 transfusion requirements 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant factor VIIa reduces transfusion requirements in liver transplant patients with high MELD scores .
	manualset3
130597	3	406053	13	NULL	NULL	0	NULL	liver transplant patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant factor VIIa reduces transfusion requirements in liver transplant patients with high MELD scores .
	manualset3
130598	4	406053	13	NULL	NULL	NULL	NULL	MELD scores	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Recombinant factor VIIa reduces transfusion requirements in liver transplant patients with high MELD scores .
	manualset3
130599	1	406054	13	NULL	NULL	0	NULL	Recombinant genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant genes can be introduced into the germ line of mice by microinjection into the fertilized egg or via embryonal carcinoma stem cells .
	manualset3
130600	2	406054	13	NULL	NULL	0	NULL	germ line	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant genes can be introduced into the germ line of mice by microinjection into the fertilized egg or via embryonal carcinoma stem cells .
	manualset3
130601	3	406054	13	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant genes can be introduced into the germ line of mice by microinjection into the fertilized egg or via embryonal carcinoma stem cells .
	manualset3
130602	4	406054	13	NULL	NULL	0	NULL	microinjection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant genes can be introduced into the germ line of mice by microinjection into the fertilized egg or via embryonal carcinoma stem cells .
	manualset3
130603	5	406054	13	NULL	NULL	0	NULL	egg 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant genes can be introduced into the germ line of mice by microinjection into the fertilized egg or via embryonal carcinoma stem cells .
	manualset3
130604	6	406054	13	NULL	NULL	0	NULL	 embryonal carcinoma stem cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant genes can be introduced into the germ line of mice by microinjection into the fertilized egg or via embryonal carcinoma stem cells .
	manualset3
130605	1	406055	13	NULL	NULL	0	NULL	Recombinant human interleukin-11 ( Neumega , rhIL-11 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant human interleukin-11 ( Neumega , rhIL-11 ) reduces thrombocytopenia in breast cancer patients receiving tandem autologous circulating progenitor cell transportation .
	manualset3
130606	2	406055	13	NULL	NULL	0	NULL	thrombocytopenia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant human interleukin-11 ( Neumega , rhIL-11 ) reduces thrombocytopenia in breast cancer patients receiving tandem autologous circulating progenitor cell transportation .
	manualset3
130607	3	406055	13	NULL	NULL	0	NULL	breast cancer patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant human interleukin-11 ( Neumega , rhIL-11 ) reduces thrombocytopenia in breast cancer patients receiving tandem autologous circulating progenitor cell transportation .
	manualset3
130608	4	406055	13	NULL	NULL	0	NULL	tandem autologous circulating progenitor cell transportation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant human interleukin-11 ( Neumega , rhIL-11 ) reduces thrombocytopenia in breast cancer patients receiving tandem autologous circulating progenitor cell transportation .
	manualset3
130609	1	406056	13	NULL	NULL	0	NULL	Recombinant human platelet-derived growth factor gel	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant human platelet-derived growth factor gel speeds healing of acute full-thickness punch biopsy wounds .
	manualset3
130610	2	406056	13	NULL	NULL	NULL	NULL	healing 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Recombinant human platelet-derived growth factor gel speeds healing of acute full-thickness punch biopsy wounds .
	manualset3
130611	3	406056	13	NULL	NULL	0	NULL	acute full-thickness punch biopsy wounds	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant human platelet-derived growth factor gel speeds healing of acute full-thickness punch biopsy wounds .
	manualset3
130612	1	406057	13	NULL	NULL	0	NULL	Recombinant human superoxide dismutase ( r-h-SOD ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant human superoxide dismutase ( r-h-SOD ) has been shown to be effective at reducing reperfusion injury , but it is not known if this infused enzyme actually reduces oxygen free radical concentrations in the myocardial tissue .
	manualset3
130613	2	406057	13	NULL	NULL	0	NULL	reperfusion injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant human superoxide dismutase ( r-h-SOD ) has been shown to be effective at reducing reperfusion injury , but it is not known if this infused enzyme actually reduces oxygen free radical concentrations in the myocardial tissue .
	manualset3
130614	3	406057	13	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant human superoxide dismutase ( r-h-SOD ) has been shown to be effective at reducing reperfusion injury , but it is not known if this infused enzyme actually reduces oxygen free radical concentrations in the myocardial tissue .
	manualset3
130615	4	406057	13	NULL	NULL	0	NULL	oxygen free radical concentrations 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant human superoxide dismutase ( r-h-SOD ) has been shown to be effective at reducing reperfusion injury , but it is not known if this infused enzyme actually reduces oxygen free radical concentrations in the myocardial tissue .
	manualset3
130616	5	406057	13	NULL	NULL	0	NULL	myocardial tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant human superoxide dismutase ( r-h-SOD ) has been shown to be effective at reducing reperfusion injury , but it is not known if this infused enzyme actually reduces oxygen free radical concentrations in the myocardial tissue .
	manualset3
130617	1	406058	13	NULL	NULL	0	NULL	Recombinant plasmids	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant plasmids containing avian vitellogenin structural gene sequences derived from complementary DNA .
	manualset3
130618	2	406058	13	NULL	NULL	0	NULL	avian vitellogenin structural gene sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant plasmids containing avian vitellogenin structural gene sequences derived from complementary DNA .
	manualset3
130619	3	406058	13	NULL	NULL	0	NULL	complementary DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant plasmids containing avian vitellogenin structural gene sequences derived from complementary DNA .
	manualset3
130620	1	406059	13	NULL	NULL	0	NULL	Recombinant vWF-A3 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant vWF-A3 was designated as a recombinant fragment comprising residues 918 - 1114 of mature vWF subunit .
	manualset3
130621	2	406059	13	NULL	NULL	0	NULL	recombinant fragment comprising residues 918 - 1114 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant vWF-A3 was designated as a recombinant fragment comprising residues 918 - 1114 of mature vWF subunit .
	manualset3
130622	3	406059	13	NULL	NULL	0	NULL	mature vWF subunit	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant vWF-A3 was designated as a recombinant fragment comprising residues 918 - 1114 of mature vWF subunit .
	manualset3
130623	1	406060	13	NULL	NULL	0	NULL	Recombination analysis results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombination analysis results revealed three recombinations among SPLCV Korea isolates , SPLCV isolates from Brazil and Japan , and ipomoea yellow vein virus ( IYVV ) Italy isolate .
	manualset3
130624	2	406060	13	NULL	NULL	0	NULL	three recombinations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombination analysis results revealed three recombinations among SPLCV Korea isolates , SPLCV isolates from Brazil and Japan , and ipomoea yellow vein virus ( IYVV ) Italy isolate .
	manualset3
130625	3	406060	13	NULL	NULL	0	NULL	SPLCV Korea isolates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombination analysis results revealed three recombinations among SPLCV Korea isolates , SPLCV isolates from Brazil and Japan , and ipomoea yellow vein virus ( IYVV ) Italy isolate .
	manualset3
130626	4	406060	13	NULL	NULL	0	NULL	SPLCV isolates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombination analysis results revealed three recombinations among SPLCV Korea isolates , SPLCV isolates from Brazil and Japan , and ipomoea yellow vein virus ( IYVV ) Italy isolate .
	manualset3
130627	5	406060	13	NULL	NULL	0	NULL	Brazil 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombination analysis results revealed three recombinations among SPLCV Korea isolates , SPLCV isolates from Brazil and Japan , and ipomoea yellow vein virus ( IYVV ) Italy isolate .
	manualset3
130628	6	406060	13	NULL	NULL	0	NULL	Japan	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombination analysis results revealed three recombinations among SPLCV Korea isolates , SPLCV isolates from Brazil and Japan , and ipomoea yellow vein virus ( IYVV ) Italy isolate .
	manualset3
130629	7	406060	13	NULL	NULL	0	NULL	ipomoea yellow vein virus ( IYVV ) Italy isolate	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombination analysis results revealed three recombinations among SPLCV Korea isolates , SPLCV isolates from Brazil and Japan , and ipomoea yellow vein virus ( IYVV ) Italy isolate .
	manualset3
130630	1	406061	13	NULL	NULL	0	NULL	Recombination	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombination and expression of Ty1 and adjacent sequences .
	manualset3
130631	2	406061	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombination and expression of Ty1 and adjacent sequences .
	manualset3
130632	3	406061	13	NULL	NULL	0	NULL	Ty1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombination and expression of Ty1 and adjacent sequences .
	manualset3
130633	4	406061	13	NULL	NULL	0	NULL	adjacent sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombination and expression of Ty1 and adjacent sequences .
	manualset3
130634	1	406062	13	NULL	NULL	0	NULL	Recombination 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombination of non-adherent spleen cells with anti-Ia and anti-Thy-1 sera treated spleen cells , however , did not restore interferon production , suggesting that other cells in addition to macrophages are depleted by the adherence procedure .
	manualset3
130635	2	406062	13	NULL	NULL	0	NULL	non-adherent spleen cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombination of non-adherent spleen cells with anti-Ia and anti-Thy-1 sera treated spleen cells , however , did not restore interferon production , suggesting that other cells in addition to macrophages are depleted by the adherence procedure .
	manualset3
130636	3	406062	13	NULL	NULL	0	NULL	anti-Ia sera treated spleen cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombination of non-adherent spleen cells with anti-Ia and anti-Thy-1 sera treated spleen cells , however , did not restore interferon production , suggesting that other cells in addition to macrophages are depleted by the adherence procedure .
	manualset3
130637	4	406062	13	NULL	NULL	0	NULL	anti-Thy-1 sera treated spleen cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombination of non-adherent spleen cells with anti-Ia and anti-Thy-1 sera treated spleen cells , however , did not restore interferon production , suggesting that other cells in addition to macrophages are depleted by the adherence procedure .
	manualset3
130638	5	406062	13	NULL	NULL	0	NULL	interferon production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombination of non-adherent spleen cells with anti-Ia and anti-Thy-1 sera treated spleen cells , however , did not restore interferon production , suggesting that other cells in addition to macrophages are depleted by the adherence procedure .
	manualset3
130639	6	406062	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombination of non-adherent spleen cells with anti-Ia and anti-Thy-1 sera treated spleen cells , however , did not restore interferon production , suggesting that other cells in addition to macrophages are depleted by the adherence procedure .
	manualset3
130640	7	406062	13	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombination of non-adherent spleen cells with anti-Ia and anti-Thy-1 sera treated spleen cells , however , did not restore interferon production , suggesting that other cells in addition to macrophages are depleted by the adherence procedure .
	manualset3
130641	8	406062	13	NULL	NULL	0	NULL	macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombination of non-adherent spleen cells with anti-Ia and anti-Thy-1 sera treated spleen cells , however , did not restore interferon production , suggesting that other cells in addition to macrophages are depleted by the adherence procedure .
	manualset3
130642	9	406062	13	NULL	NULL	0	NULL	adherence procedure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombination of non-adherent spleen cells with anti-Ia and anti-Thy-1 sera treated spleen cells , however , did not restore interferon production , suggesting that other cells in addition to macrophages are depleted by the adherence procedure .
	manualset3
130643	1	406063	13	NULL	NULL	0	NULL	Recommendations	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Recommendations for rescue therapy of breakthrough PONV are also provided .
	manualset3
130644	2	406063	13	NULL	NULL	0	NULL	rescue therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recommendations for rescue therapy of breakthrough PONV are also provided .
	manualset3
130645	3	406063	13	NULL	NULL	0	NULL	breakthrough PONV	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recommendations for rescue therapy of breakthrough PONV are also provided .
	manualset3
130646	1	406064	13	NULL	NULL	0	NULL	Recommendations	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Recommendations for translation and reliability testing of International Spinal Cord Injury Data Sets .
	manualset3
130647	2	406064	13	NULL	NULL	NULL	NULL	translation 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Recommendations for translation and reliability testing of International Spinal Cord Injury Data Sets .
	manualset3
130648	3	406064	13	NULL	NULL	0	NULL	reliability testing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recommendations for translation and reliability testing of International Spinal Cord Injury Data Sets .
	manualset3
130649	4	406064	13	NULL	NULL	0	NULL	International Spinal Cord Injury Data Sets	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Recommendations for translation and reliability testing of International Spinal Cord Injury Data Sets .
	manualset3
130650	1	406065	13	NULL	NULL	0	NULL	Recommendations	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Recommendations include assessing suicide risk regularly throughout hospitalization , including on admission , during changes in a patient 's mental or physical status , after a change in observation level , and before discharge .
	manualset3
130651	2	406065	13	NULL	NULL	0	NULL	suicide risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recommendations include assessing suicide risk regularly throughout hospitalization , including on admission , during changes in a patient 's mental or physical status , after a change in observation level , and before discharge .
	manualset3
130652	3	406065	13	NULL	NULL	0	NULL	hospitalization 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recommendations include assessing suicide risk regularly throughout hospitalization , including on admission , during changes in a patient 's mental or physical status , after a change in observation level , and before discharge .
	manualset3
130653	4	406065	13	NULL	NULL	0	NULL	admission	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recommendations include assessing suicide risk regularly throughout hospitalization , including on admission , during changes in a patient 's mental or physical status , after a change in observation level , and before discharge .
	manualset3
130654	5	406065	13	NULL	NULL	0	NULL	changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recommendations include assessing suicide risk regularly throughout hospitalization , including on admission , during changes in a patient 's mental or physical status , after a change in observation level , and before discharge .
	manualset3
130655	6	406065	13	NULL	NULL	0	NULL	patient 's mental status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recommendations include assessing suicide risk regularly throughout hospitalization , including on admission , during changes in a patient 's mental or physical status , after a change in observation level , and before discharge .
	manualset3
130656	7	406065	13	NULL	NULL	0	NULL	patient 's physical status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recommendations include assessing suicide risk regularly throughout hospitalization , including on admission , during changes in a patient 's mental or physical status , after a change in observation level , and before discharge .
	manualset3
130657	8	406065	13	NULL	NULL	0	NULL	change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recommendations include assessing suicide risk regularly throughout hospitalization , including on admission , during changes in a patient 's mental or physical status , after a change in observation level , and before discharge .
	manualset3
130658	9	406065	13	NULL	NULL	0	NULL	observation level	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recommendations include assessing suicide risk regularly throughout hospitalization , including on admission , during changes in a patient 's mental or physical status , after a change in observation level , and before discharge .
	manualset3
130659	10	406065	13	NULL	NULL	0	NULL	discharge	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recommendations include assessing suicide risk regularly throughout hospitalization , including on admission , during changes in a patient 's mental or physical status , after a change in observation level , and before discharge .
	manualset3
130660	1	406066	13	NULL	NULL	0	NULL	Recommendations	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Recommendations promoting the use of cost-effective anti-inflammatory medications are crucial to efficiently managing asthma .
	manualset3
130661	2	406066	13	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recommendations promoting the use of cost-effective anti-inflammatory medications are crucial to efficiently managing asthma .
	manualset3
130662	3	406066	13	NULL	NULL	0	NULL	 cost-effective anti-inflammatory medications 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Recommendations promoting the use of cost-effective anti-inflammatory medications are crucial to efficiently managing asthma .
	manualset3
130663	4	406066	13	NULL	NULL	0	NULL	asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Recommendations promoting the use of cost-effective anti-inflammatory medications are crucial to efficiently managing asthma .
	manualset3
130664	1	406067	13	NULL	NULL	0	NULL	Reconstitution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reconstitution of Raf-1 activity was observed only with kinase active Jak1 in both cell lines .
	manualset3
130665	2	406067	13	NULL	NULL	0	NULL	Raf-1 activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reconstitution of Raf-1 activity was observed only with kinase active Jak1 in both cell lines .
	manualset3
130666	3	406067	13	NULL	NULL	0	NULL	kinase active Jak1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Reconstitution of Raf-1 activity was observed only with kinase active Jak1 in both cell lines .
	manualset3
130667	4	406067	13	NULL	NULL	0	NULL	both cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Reconstitution of Raf-1 activity was observed only with kinase active Jak1 in both cell lines .
	manualset3
130668	1	406068	13	NULL	NULL	0	NULL	Reconstitution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reconstitution of contractile FtsZ rings in liposomes .
	manualset3
130669	2	406068	13	NULL	NULL	0	NULL	FtsZ rings	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Reconstitution of contractile FtsZ rings in liposomes .
	manualset3
130670	3	406068	13	NULL	NULL	0	NULL	liposomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Reconstitution of contractile FtsZ rings in liposomes .
	manualset3
130671	1	406069	13	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A model based on results provided by evidence-based medicine suggested that a `` polypill '' , that contains a statin , three blood pressure lowering drugs ( each at half standard dose ) , aspirin and folic acid , would result in an 80 % reduction in the incidence of coronary and cerebrovascular events , while being associated with a good tolerance profile and offering a favourable cost-effectiveness ratio .
	manualset3
130672	2	406069	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A model based on results provided by evidence-based medicine suggested that a `` polypill '' , that contains a statin , three blood pressure lowering drugs ( each at half standard dose ) , aspirin and folic acid , would result in an 80 % reduction in the incidence of coronary and cerebrovascular events , while being associated with a good tolerance profile and offering a favourable cost-effectiveness ratio .
	manualset3
130673	3	406069	13	NULL	NULL	0	NULL	evidence-based medicine	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A model based on results provided by evidence-based medicine suggested that a `` polypill '' , that contains a statin , three blood pressure lowering drugs ( each at half standard dose ) , aspirin and folic acid , would result in an 80 % reduction in the incidence of coronary and cerebrovascular events , while being associated with a good tolerance profile and offering a favourable cost-effectiveness ratio .
	manualset3
130674	4	406069	13	NULL	NULL	0	NULL	polypill	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A model based on results provided by evidence-based medicine suggested that a `` polypill '' , that contains a statin , three blood pressure lowering drugs ( each at half standard dose ) , aspirin and folic acid , would result in an 80 % reduction in the incidence of coronary and cerebrovascular events , while being associated with a good tolerance profile and offering a favourable cost-effectiveness ratio .
	manualset3
130675	5	406069	13	NULL	NULL	0	NULL	statin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A model based on results provided by evidence-based medicine suggested that a `` polypill '' , that contains a statin , three blood pressure lowering drugs ( each at half standard dose ) , aspirin and folic acid , would result in an 80 % reduction in the incidence of coronary and cerebrovascular events , while being associated with a good tolerance profile and offering a favourable cost-effectiveness ratio .
	manualset3
130676	6	406069	13	NULL	NULL	0	NULL	three blood pressure lowering drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A model based on results provided by evidence-based medicine suggested that a `` polypill '' , that contains a statin , three blood pressure lowering drugs ( each at half standard dose ) , aspirin and folic acid , would result in an 80 % reduction in the incidence of coronary and cerebrovascular events , while being associated with a good tolerance profile and offering a favourable cost-effectiveness ratio .
	manualset3
130677	7	406069	13	NULL	NULL	0	NULL	half standard dose	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A model based on results provided by evidence-based medicine suggested that a `` polypill '' , that contains a statin , three blood pressure lowering drugs ( each at half standard dose ) , aspirin and folic acid , would result in an 80 % reduction in the incidence of coronary and cerebrovascular events , while being associated with a good tolerance profile and offering a favourable cost-effectiveness ratio .
	manualset3
130678	8	406069	13	NULL	NULL	0	NULL	aspirin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A model based on results provided by evidence-based medicine suggested that a `` polypill '' , that contains a statin , three blood pressure lowering drugs ( each at half standard dose ) , aspirin and folic acid , would result in an 80 % reduction in the incidence of coronary and cerebrovascular events , while being associated with a good tolerance profile and offering a favourable cost-effectiveness ratio .
	manualset3
130679	9	406069	13	NULL	NULL	0	NULL	folic acid	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A model based on results provided by evidence-based medicine suggested that a `` polypill '' , that contains a statin , three blood pressure lowering drugs ( each at half standard dose ) , aspirin and folic acid , would result in an 80 % reduction in the incidence of coronary and cerebrovascular events , while being associated with a good tolerance profile and offering a favourable cost-effectiveness ratio .
	manualset3
130680	10	406069	13	NULL	NULL	0	NULL	80 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A model based on results provided by evidence-based medicine suggested that a `` polypill '' , that contains a statin , three blood pressure lowering drugs ( each at half standard dose ) , aspirin and folic acid , would result in an 80 % reduction in the incidence of coronary and cerebrovascular events , while being associated with a good tolerance profile and offering a favourable cost-effectiveness ratio .
	manualset3
130681	11	406069	13	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A model based on results provided by evidence-based medicine suggested that a `` polypill '' , that contains a statin , three blood pressure lowering drugs ( each at half standard dose ) , aspirin and folic acid , would result in an 80 % reduction in the incidence of coronary and cerebrovascular events , while being associated with a good tolerance profile and offering a favourable cost-effectiveness ratio .
	manualset3
130682	12	406069	13	NULL	NULL	0	NULL	incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A model based on results provided by evidence-based medicine suggested that a `` polypill '' , that contains a statin , three blood pressure lowering drugs ( each at half standard dose ) , aspirin and folic acid , would result in an 80 % reduction in the incidence of coronary and cerebrovascular events , while being associated with a good tolerance profile and offering a favourable cost-effectiveness ratio .
	manualset3
130683	13	406069	13	NULL	NULL	0	NULL	coronary events	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A model based on results provided by evidence-based medicine suggested that a `` polypill '' , that contains a statin , three blood pressure lowering drugs ( each at half standard dose ) , aspirin and folic acid , would result in an 80 % reduction in the incidence of coronary and cerebrovascular events , while being associated with a good tolerance profile and offering a favourable cost-effectiveness ratio .
	manualset3
130684	14	406069	13	NULL	NULL	0	NULL	cerebrovascular events	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A model based on results provided by evidence-based medicine suggested that a `` polypill '' , that contains a statin , three blood pressure lowering drugs ( each at half standard dose ) , aspirin and folic acid , would result in an 80 % reduction in the incidence of coronary and cerebrovascular events , while being associated with a good tolerance profile and offering a favourable cost-effectiveness ratio .
	manualset3
130685	15	406069	13	NULL	NULL	0	NULL	good tolerance profile 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A model based on results provided by evidence-based medicine suggested that a `` polypill '' , that contains a statin , three blood pressure lowering drugs ( each at half standard dose ) , aspirin and folic acid , would result in an 80 % reduction in the incidence of coronary and cerebrovascular events , while being associated with a good tolerance profile and offering a favourable cost-effectiveness ratio .
	manualset3
130686	16	406069	13	NULL	NULL	0	NULL	cost-effectiveness ratio	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A model based on results provided by evidence-based medicine suggested that a `` polypill '' , that contains a statin , three blood pressure lowering drugs ( each at half standard dose ) , aspirin and folic acid , would result in an 80 % reduction in the incidence of coronary and cerebrovascular events , while being associated with a good tolerance profile and offering a favourable cost-effectiveness ratio .
	manualset3
130687	1	406070	13	NULL	NULL	0	NULL	Reconstructing stimuli	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reconstructing stimuli from the spike times of leaky integrate and fire neurons .
	manualset3
130688	2	406070	13	NULL	NULL	0	NULL	spike times	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reconstructing stimuli from the spike times of leaky integrate and fire neurons .
	manualset3
130689	3	406070	13	NULL	NULL	0	NULL	leaky integrate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reconstructing stimuli from the spike times of leaky integrate and fire neurons .
	manualset3
130690	4	406070	13	NULL	NULL	0	NULL	fire neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Reconstructing stimuli from the spike times of leaky integrate and fire neurons .
	manualset3
130691	1	406071	13	NULL	NULL	0	NULL	Reconstruction plate	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Reconstruction plate was used in seven patients and tension band wiring in just one .
	manualset3
130692	2	406071	13	NULL	NULL	0	NULL	seven patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Reconstruction plate was used in seven patients and tension band wiring in just one .
	manualset3
130693	3	406071	13	NULL	NULL	0	NULL	tension band wiring 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Reconstruction plate was used in seven patients and tension band wiring in just one .
	manualset3
134806	4	406071	13	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Reconstruction plate was used in seven patients and tension band wiring in just one .
	manualset3
130694	1	406072	13	NULL	NULL	0	NULL	karyometric parameters	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recorded karyometric and histometric parameters include measures of nuclear DNA content ( based on optical density measurements ) , size , roundness , texture , shape , distance to the basal layer , angle with the stratum germinativum , epithelial height and proximate nuclear distance .
	manualset3
130695	2	406072	13	NULL	NULL	0	NULL	histometric parameters	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recorded karyometric and histometric parameters include measures of nuclear DNA content ( based on optical density measurements ) , size , roundness , texture , shape , distance to the basal layer , angle with the stratum germinativum , epithelial height and proximate nuclear distance .
	manualset3
130696	3	406072	13	NULL	NULL	0	NULL	measures 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recorded karyometric and histometric parameters include measures of nuclear DNA content ( based on optical density measurements ) , size , roundness , texture , shape , distance to the basal layer , angle with the stratum germinativum , epithelial height and proximate nuclear distance .
	manualset3
130697	4	406072	13	NULL	NULL	0	NULL	nuclear DNA content	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recorded karyometric and histometric parameters include measures of nuclear DNA content ( based on optical density measurements ) , size , roundness , texture , shape , distance to the basal layer , angle with the stratum germinativum , epithelial height and proximate nuclear distance .
	manualset3
130698	5	406072	13	NULL	NULL	0	NULL	optical density measurements	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recorded karyometric and histometric parameters include measures of nuclear DNA content ( based on optical density measurements ) , size , roundness , texture , shape , distance to the basal layer , angle with the stratum germinativum , epithelial height and proximate nuclear distance .
	manualset3
130699	6	406072	13	NULL	NULL	0	NULL	size	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recorded karyometric and histometric parameters include measures of nuclear DNA content ( based on optical density measurements ) , size , roundness , texture , shape , distance to the basal layer , angle with the stratum germinativum , epithelial height and proximate nuclear distance .
	manualset3
130700	7	406072	13	NULL	NULL	0	NULL	roundness	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recorded karyometric and histometric parameters include measures of nuclear DNA content ( based on optical density measurements ) , size , roundness , texture , shape , distance to the basal layer , angle with the stratum germinativum , epithelial height and proximate nuclear distance .
	manualset3
130701	8	406072	13	NULL	NULL	0	NULL	texture	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recorded karyometric and histometric parameters include measures of nuclear DNA content ( based on optical density measurements ) , size , roundness , texture , shape , distance to the basal layer , angle with the stratum germinativum , epithelial height and proximate nuclear distance .
	manualset3
130702	9	406072	13	NULL	NULL	0	NULL	shape	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recorded karyometric and histometric parameters include measures of nuclear DNA content ( based on optical density measurements ) , size , roundness , texture , shape , distance to the basal layer , angle with the stratum germinativum , epithelial height and proximate nuclear distance .
	manualset3
130703	10	406072	13	NULL	NULL	0	NULL	distance	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recorded karyometric and histometric parameters include measures of nuclear DNA content ( based on optical density measurements ) , size , roundness , texture , shape , distance to the basal layer , angle with the stratum germinativum , epithelial height and proximate nuclear distance .
	manualset3
130704	11	406072	13	NULL	NULL	0	NULL	basal layer	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Recorded karyometric and histometric parameters include measures of nuclear DNA content ( based on optical density measurements ) , size , roundness , texture , shape , distance to the basal layer , angle with the stratum germinativum , epithelial height and proximate nuclear distance .
	manualset3
130705	12	406072	13	NULL	NULL	0	NULL	angle	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recorded karyometric and histometric parameters include measures of nuclear DNA content ( based on optical density measurements ) , size , roundness , texture , shape , distance to the basal layer , angle with the stratum germinativum , epithelial height and proximate nuclear distance .
	manualset3
130706	13	406072	13	NULL	NULL	0	NULL	stratum germinativum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Recorded karyometric and histometric parameters include measures of nuclear DNA content ( based on optical density measurements ) , size , roundness , texture , shape , distance to the basal layer , angle with the stratum germinativum , epithelial height and proximate nuclear distance .
	manualset3
130707	14	406072	13	NULL	NULL	0	NULL	epithelial height 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recorded karyometric and histometric parameters include measures of nuclear DNA content ( based on optical density measurements ) , size , roundness , texture , shape , distance to the basal layer , angle with the stratum germinativum , epithelial height and proximate nuclear distance .
	manualset3
130708	15	406072	13	NULL	NULL	0	NULL	proximate nuclear distance 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recorded karyometric and histometric parameters include measures of nuclear DNA content ( based on optical density measurements ) , size , roundness , texture , shape , distance to the basal layer , angle with the stratum germinativum , epithelial height and proximate nuclear distance .
	manualset3
130709	1	406073	13	NULL	NULL	0	NULL	Recoveries	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recoveries at the limit of quantitation were between 75 and 95 % for both analytes , with a 4.8-9 .3 % range in standard deviation .
	manualset3
130710	2	406073	13	NULL	NULL	0	NULL	limit of quantitation	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recoveries at the limit of quantitation were between 75 and 95 % for both analytes , with a 4.8-9 .3 % range in standard deviation .
	manualset3
130711	3	406073	13	NULL	NULL	0	NULL	between 75 and 95 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recoveries at the limit of quantitation were between 75 and 95 % for both analytes , with a 4.8-9 .3 % range in standard deviation .
	manualset3
130712	4	406073	13	NULL	NULL	0	NULL	analytes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Recoveries at the limit of quantitation were between 75 and 95 % for both analytes , with a 4.8-9 .3 % range in standard deviation .
	manualset3
130713	5	406073	13	NULL	NULL	0	NULL	 4.8-9 .3 % range	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recoveries at the limit of quantitation were between 75 and 95 % for both analytes , with a 4.8-9 .3 % range in standard deviation .
	manualset3
130714	6	406073	13	NULL	NULL	0	NULL	standard deviation	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recoveries at the limit of quantitation were between 75 and 95 % for both analytes , with a 4.8-9 .3 % range in standard deviation .
	manualset3
130715	1	406074	13	NULL	NULL	0	NULL	Recovery 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery and purity were significantly improved upon adaptation of the hybridoma to serum-free media .
	manualset3
130716	2	406074	13	NULL	NULL	0	NULL	purity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery and purity were significantly improved upon adaptation of the hybridoma to serum-free media .
	manualset3
130717	3	406074	13	NULL	NULL	0	NULL	adaptation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery and purity were significantly improved upon adaptation of the hybridoma to serum-free media .
	manualset3
130718	4	406074	13	NULL	NULL	0	NULL	hybridoma	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery and purity were significantly improved upon adaptation of the hybridoma to serum-free media .
	manualset3
130719	5	406074	13	NULL	NULL	0	NULL	serum-free media	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery and purity were significantly improved upon adaptation of the hybridoma to serum-free media .
	manualset3
130720	1	406075	13	NULL	NULL	0	NULL	Recovery	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery from drought stress in tobacco : an active process associated with the reversal of senescence in some plant parts and the sacrifice of others .
	manualset3
130721	2	406075	13	NULL	NULL	0	NULL	drought stress	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery from drought stress in tobacco : an active process associated with the reversal of senescence in some plant parts and the sacrifice of others .
	manualset3
130722	3	406075	13	NULL	NULL	0	NULL	tobacco	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery from drought stress in tobacco : an active process associated with the reversal of senescence in some plant parts and the sacrifice of others .
	manualset3
130723	4	406075	13	NULL	NULL	0	NULL	active process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery from drought stress in tobacco : an active process associated with the reversal of senescence in some plant parts and the sacrifice of others .
	manualset3
130724	5	406075	13	NULL	NULL	0	NULL	reversal 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery from drought stress in tobacco : an active process associated with the reversal of senescence in some plant parts and the sacrifice of others .
	manualset3
130725	6	406075	13	NULL	NULL	0	NULL	senescence 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery from drought stress in tobacco : an active process associated with the reversal of senescence in some plant parts and the sacrifice of others .
	manualset3
130726	7	406075	13	NULL	NULL	0	NULL	plant parts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery from drought stress in tobacco : an active process associated with the reversal of senescence in some plant parts and the sacrifice of others .
	manualset3
130727	8	406075	13	NULL	NULL	0	NULL	sacrifice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery from drought stress in tobacco : an active process associated with the reversal of senescence in some plant parts and the sacrifice of others .
	manualset3
130728	9	406075	13	NULL	NULL	0	NULL	others	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery from drought stress in tobacco : an active process associated with the reversal of senescence in some plant parts and the sacrifice of others .
	manualset3
130729	1	406076	13	NULL	NULL	0	NULL	Recovery 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery from substance use is a vital concern for many women with human immunodeficiency virus ( HIV ) / acquired immune deficiency syndrome ( AIDS ) .
	manualset3
130730	2	406076	13	NULL	NULL	0	NULL	substance use	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery from substance use is a vital concern for many women with human immunodeficiency virus ( HIV ) / acquired immune deficiency syndrome ( AIDS ) .
	manualset3
130731	3	406076	13	NULL	NULL	0	NULL	concern	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery from substance use is a vital concern for many women with human immunodeficiency virus ( HIV ) / acquired immune deficiency syndrome ( AIDS ) .
	manualset3
130732	4	406076	13	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery from substance use is a vital concern for many women with human immunodeficiency virus ( HIV ) / acquired immune deficiency syndrome ( AIDS ) .
	manualset3
130733	5	406076	13	NULL	NULL	0	NULL	human immunodeficiency virus ( HIV ) / acquired immune deficiency syndrome ( AIDS )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery from substance use is a vital concern for many women with human immunodeficiency virus ( HIV ) / acquired immune deficiency syndrome ( AIDS ) .
	manualset3
130734	1	406077	13	NULL	NULL	0	NULL	Recovery	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery of contractile function was unrelated to pH ( i ) during ischemia ; the glucose-perfused control and palmitate-perfused diabetic hearts had end-ischemic pH ( i ) values that were significantly different at 6.36 + / - 0.04 and 6.60 + / - 0.02 , respectively , but had similar functional recoveries , whereas the glucose-perfused diabetic hearts had significantly lower functional recoveries , but their pH ( i ) was 6.49 + / - 0.04 .
	manualset3
130735	2	406077	13	NULL	NULL	0	NULL	contractile function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery of contractile function was unrelated to pH ( i ) during ischemia ; the glucose-perfused control and palmitate-perfused diabetic hearts had end-ischemic pH ( i ) values that were significantly different at 6.36 + / - 0.04 and 6.60 + / - 0.02 , respectively , but had similar functional recoveries , whereas the glucose-perfused diabetic hearts had significantly lower functional recoveries , but their pH ( i ) was 6.49 + / - 0.04 .
	manualset3
130736	3	406077	13	NULL	NULL	0	NULL	pH 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery of contractile function was unrelated to pH ( i ) during ischemia ; the glucose-perfused control and palmitate-perfused diabetic hearts had end-ischemic pH ( i ) values that were significantly different at 6.36 + / - 0.04 and 6.60 + / - 0.02 , respectively , but had similar functional recoveries , whereas the glucose-perfused diabetic hearts had significantly lower functional recoveries , but their pH ( i ) was 6.49 + / - 0.04 .
	manualset3
130737	4	406077	13	NULL	NULL	0	NULL	ischemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery of contractile function was unrelated to pH ( i ) during ischemia ; the glucose-perfused control and palmitate-perfused diabetic hearts had end-ischemic pH ( i ) values that were significantly different at 6.36 + / - 0.04 and 6.60 + / - 0.02 , respectively , but had similar functional recoveries , whereas the glucose-perfused diabetic hearts had significantly lower functional recoveries , but their pH ( i ) was 6.49 + / - 0.04 .
	manualset3
130738	5	406077	13	NULL	NULL	0	NULL	glucose-perfused control	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery of contractile function was unrelated to pH ( i ) during ischemia ; the glucose-perfused control and palmitate-perfused diabetic hearts had end-ischemic pH ( i ) values that were significantly different at 6.36 + / - 0.04 and 6.60 + / - 0.02 , respectively , but had similar functional recoveries , whereas the glucose-perfused diabetic hearts had significantly lower functional recoveries , but their pH ( i ) was 6.49 + / - 0.04 .
	manualset3
130739	6	406077	13	NULL	NULL	0	NULL	palmitate-perfused diabetic hearts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery of contractile function was unrelated to pH ( i ) during ischemia ; the glucose-perfused control and palmitate-perfused diabetic hearts had end-ischemic pH ( i ) values that were significantly different at 6.36 + / - 0.04 and 6.60 + / - 0.02 , respectively , but had similar functional recoveries , whereas the glucose-perfused diabetic hearts had significantly lower functional recoveries , but their pH ( i ) was 6.49 + / - 0.04 .
	manualset3
130740	7	406077	13	NULL	NULL	0	NULL	end-ischemic pH ( i ) values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery of contractile function was unrelated to pH ( i ) during ischemia ; the glucose-perfused control and palmitate-perfused diabetic hearts had end-ischemic pH ( i ) values that were significantly different at 6.36 + / - 0.04 and 6.60 + / - 0.02 , respectively , but had similar functional recoveries , whereas the glucose-perfused diabetic hearts had significantly lower functional recoveries , but their pH ( i ) was 6.49 + / - 0.04 .
	manualset3
130741	8	406077	13	NULL	NULL	0	NULL	6.36 + / - 0.04	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery of contractile function was unrelated to pH ( i ) during ischemia ; the glucose-perfused control and palmitate-perfused diabetic hearts had end-ischemic pH ( i ) values that were significantly different at 6.36 + / - 0.04 and 6.60 + / - 0.02 , respectively , but had similar functional recoveries , whereas the glucose-perfused diabetic hearts had significantly lower functional recoveries , but their pH ( i ) was 6.49 + / - 0.04 .
	manualset3
130742	9	406077	13	NULL	NULL	0	NULL	6.60 + / - 0.02	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery of contractile function was unrelated to pH ( i ) during ischemia ; the glucose-perfused control and palmitate-perfused diabetic hearts had end-ischemic pH ( i ) values that were significantly different at 6.36 + / - 0.04 and 6.60 + / - 0.02 , respectively , but had similar functional recoveries , whereas the glucose-perfused diabetic hearts had significantly lower functional recoveries , but their pH ( i ) was 6.49 + / - 0.04 .
	manualset3
130743	10	406077	13	NULL	NULL	0	NULL	functional recoveries 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery of contractile function was unrelated to pH ( i ) during ischemia ; the glucose-perfused control and palmitate-perfused diabetic hearts had end-ischemic pH ( i ) values that were significantly different at 6.36 + / - 0.04 and 6.60 + / - 0.02 , respectively , but had similar functional recoveries , whereas the glucose-perfused diabetic hearts had significantly lower functional recoveries , but their pH ( i ) was 6.49 + / - 0.04 .
	manualset3
130744	11	406077	13	NULL	NULL	0	NULL	 glucose-perfused diabetic hearts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery of contractile function was unrelated to pH ( i ) during ischemia ; the glucose-perfused control and palmitate-perfused diabetic hearts had end-ischemic pH ( i ) values that were significantly different at 6.36 + / - 0.04 and 6.60 + / - 0.02 , respectively , but had similar functional recoveries , whereas the glucose-perfused diabetic hearts had significantly lower functional recoveries , but their pH ( i ) was 6.49 + / - 0.04 .
	manualset3
130745	12	406077	13	NULL	NULL	0	NULL	functional recoveries 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery of contractile function was unrelated to pH ( i ) during ischemia ; the glucose-perfused control and palmitate-perfused diabetic hearts had end-ischemic pH ( i ) values that were significantly different at 6.36 + / - 0.04 and 6.60 + / - 0.02 , respectively , but had similar functional recoveries , whereas the glucose-perfused diabetic hearts had significantly lower functional recoveries , but their pH ( i ) was 6.49 + / - 0.04 .
	manualset3
130746	13	406077	13	NULL	NULL	0	NULL	 pH ( i )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery of contractile function was unrelated to pH ( i ) during ischemia ; the glucose-perfused control and palmitate-perfused diabetic hearts had end-ischemic pH ( i ) values that were significantly different at 6.36 + / - 0.04 and 6.60 + / - 0.02 , respectively , but had similar functional recoveries , whereas the glucose-perfused diabetic hearts had significantly lower functional recoveries , but their pH ( i ) was 6.49 + / - 0.04 .
	manualset3
130747	14	406077	13	NULL	NULL	0	NULL	6.49 + / - 0.04	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery of contractile function was unrelated to pH ( i ) during ischemia ; the glucose-perfused control and palmitate-perfused diabetic hearts had end-ischemic pH ( i ) values that were significantly different at 6.36 + / - 0.04 and 6.60 + / - 0.02 , respectively , but had similar functional recoveries , whereas the glucose-perfused diabetic hearts had significantly lower functional recoveries , but their pH ( i ) was 6.49 + / - 0.04 .
	manualset3
130748	1	406078	13	NULL	NULL	NULL	NULL	Recovery 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Recovery of functional cytotoxic T lymphocytes during lamivudine therapy by acquiring multi-specificity .
	manualset3
130749	2	406078	13	NULL	NULL	0	NULL	functional cytotoxic T lymphocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery of functional cytotoxic T lymphocytes during lamivudine therapy by acquiring multi-specificity .
	manualset3
130750	3	406078	13	NULL	NULL	0	NULL	lamivudine therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery of functional cytotoxic T lymphocytes during lamivudine therapy by acquiring multi-specificity .
	manualset3
130751	4	406078	13	NULL	NULL	0	NULL	multi-specificity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recovery of functional cytotoxic T lymphocytes during lamivudine therapy by acquiring multi-specificity .
	manualset3
130752	1	406079	13	NULL	NULL	0	NULL	Recreational values 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recreational values of a nursing school library .
	manualset3
130753	2	406079	13	NULL	NULL	0	NULL	nursing school library	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Recreational values of a nursing school library .
	manualset3
130754	1	406080	13	NULL	NULL	0	NULL	Rectal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Rectal cancer : the influence of tumor proliferation on response to preoperative irradiation .
	manualset3
130755	2	406080	13	NULL	NULL	0	NULL	influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rectal cancer : the influence of tumor proliferation on response to preoperative irradiation .
	manualset3
130756	3	406080	13	NULL	NULL	0	NULL	tumor proliferation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rectal cancer : the influence of tumor proliferation on response to preoperative irradiation .
	manualset3
130757	4	406080	13	NULL	NULL	0	NULL	response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rectal cancer : the influence of tumor proliferation on response to preoperative irradiation .
	manualset3
130758	5	406080	13	NULL	NULL	0	NULL	preoperative irradiation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Rectal cancer : the influence of tumor proliferation on response to preoperative irradiation .
	manualset3
130759	1	406081	13	NULL	NULL	0	NULL	Recurrent digital ulnar deviation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recurrent digital ulnar deviation was observed in 58 % of patients , digital malrotation in 50 % , and extensor tendon redislocation in 45 % .
	manualset3
130760	2	406081	13	NULL	NULL	0	NULL	58 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recurrent digital ulnar deviation was observed in 58 % of patients , digital malrotation in 50 % , and extensor tendon redislocation in 45 % .
	manualset3
130761	3	406081	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recurrent digital ulnar deviation was observed in 58 % of patients , digital malrotation in 50 % , and extensor tendon redislocation in 45 % .
	manualset3
130762	4	406081	13	NULL	NULL	0	NULL	digital malrotation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recurrent digital ulnar deviation was observed in 58 % of patients , digital malrotation in 50 % , and extensor tendon redislocation in 45 % .
	manualset3
130763	5	406081	13	NULL	NULL	0	NULL	50 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recurrent digital ulnar deviation was observed in 58 % of patients , digital malrotation in 50 % , and extensor tendon redislocation in 45 % .
	manualset3
130764	6	406081	13	NULL	NULL	0	NULL	extensor tendon redislocation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recurrent digital ulnar deviation was observed in 58 % of patients , digital malrotation in 50 % , and extensor tendon redislocation in 45 % .
	manualset3
130765	7	406081	13	NULL	NULL	0	NULL	45 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Recurrent digital ulnar deviation was observed in 58 % of patients , digital malrotation in 50 % , and extensor tendon redislocation in 45 % .
	manualset3
130766	1	406082	13	NULL	NULL	0	NULL	Recurrent pulmonary edema 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recurrent pulmonary edema caused by chronic left main coronary artery occlusion .
	manualset3
130767	2	406082	13	NULL	NULL	0	NULL	chronic left main coronary artery occlusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recurrent pulmonary edema caused by chronic left main coronary artery occlusion .
	manualset3
130768	1	406083	13	NULL	NULL	0	NULL	Recurrent squamous cell carcinoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recurrent squamous cell carcinoma presenting as facial nerve palsy in the setting of organ transplantation .
	manualset3
130769	2	406083	13	NULL	NULL	0	NULL	facial nerve palsy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recurrent squamous cell carcinoma presenting as facial nerve palsy in the setting of organ transplantation .
	manualset3
130770	3	406083	13	NULL	NULL	NULL	NULL	setting of organ transplantation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Recurrent squamous cell carcinoma presenting as facial nerve palsy in the setting of organ transplantation .
	manualset3
130771	1	406084	13	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A model for the differentiation of human natural killer cells .
	manualset3
130772	2	406084	13	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A model for the differentiation of human natural killer cells .
	manualset3
130773	3	406084	13	NULL	NULL	0	NULL	human natural killer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A model for the differentiation of human natural killer cells .
	manualset3
130774	1	406085	13	NULL	NULL	0	NULL	Red blood cell volume	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Red blood cell volume and plasma volume were determined by using chromium-51-tagged erythrocytes and iodine-125-labeled albumin , respectively .
	manualset3
130775	2	406085	13	NULL	NULL	NULL	NULL	plasma volume	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Red blood cell volume and plasma volume were determined by using chromium-51-tagged erythrocytes and iodine-125-labeled albumin , respectively .
	manualset3
130776	3	406085	13	NULL	NULL	0	NULL	chromium-51-tagged erythrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Red blood cell volume and plasma volume were determined by using chromium-51-tagged erythrocytes and iodine-125-labeled albumin , respectively .
	manualset3
130777	4	406085	13	NULL	NULL	0	NULL	iodine-125-labeled albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Red blood cell volume and plasma volume were determined by using chromium-51-tagged erythrocytes and iodine-125-labeled albumin , respectively .
	manualset3
130778	1	406086	13	NULL	NULL	0	NULL	Red yeast rice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Red yeast rice to treat cholesterol problems in patients who can not tolerate statin therapy because of muscle pain .
	manualset3
130779	2	406086	13	NULL	NULL	0	NULL	cholesterol problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Red yeast rice to treat cholesterol problems in patients who can not tolerate statin therapy because of muscle pain .
	manualset3
130780	3	406086	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Red yeast rice to treat cholesterol problems in patients who can not tolerate statin therapy because of muscle pain .
	manualset3
130781	4	406086	13	NULL	NULL	0	NULL	statin therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Red yeast rice to treat cholesterol problems in patients who can not tolerate statin therapy because of muscle pain .
	manualset3
130782	5	406086	13	NULL	NULL	0	NULL	muscle pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Red yeast rice to treat cholesterol problems in patients who can not tolerate statin therapy because of muscle pain .
	manualset3
130783	1	406087	13	NULL	NULL	0	NULL	Rediscovery	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rediscovery of Trichinella spiralis in red foxes ( Vulpes vulpes ) in Ireland after 30 years of oblivion .
	manualset3
130784	2	406087	13	NULL	NULL	0	NULL	Trichinella spiralis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rediscovery of Trichinella spiralis in red foxes ( Vulpes vulpes ) in Ireland after 30 years of oblivion .
	manualset3
130785	3	406087	13	NULL	NULL	0	NULL	red foxes ( Vulpes vulpes )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rediscovery of Trichinella spiralis in red foxes ( Vulpes vulpes ) in Ireland after 30 years of oblivion .
	manualset3
130786	4	406087	13	NULL	NULL	0	NULL	Ireland	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Rediscovery of Trichinella spiralis in red foxes ( Vulpes vulpes ) in Ireland after 30 years of oblivion .
	manualset3
130787	5	406087	13	NULL	NULL	0	NULL	30 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Rediscovery of Trichinella spiralis in red foxes ( Vulpes vulpes ) in Ireland after 30 years of oblivion .
	manualset3
130788	6	406087	13	NULL	NULL	0	NULL	oblivion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rediscovery of Trichinella spiralis in red foxes ( Vulpes vulpes ) in Ireland after 30 years of oblivion .
	manualset3
130789	1	406088	13	NULL	NULL	0	NULL	Redox-dependent conformational changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Redox-dependent conformational changes of bovine Cu , Zn superoxide dismutase in 20 mM phosphate buffer ( pH 7.4 ) were studied at 20 degrees C using Fourier transform infrared spectroscopy .
	manualset3
130790	2	406088	13	NULL	NULL	0	NULL	bovine Cu , Zn superoxide dismutase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Redox-dependent conformational changes of bovine Cu , Zn superoxide dismutase in 20 mM phosphate buffer ( pH 7.4 ) were studied at 20 degrees C using Fourier transform infrared spectroscopy .
	manualset3
130791	3	406088	13	NULL	NULL	0	NULL	20 mM phosphate buffer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Redox-dependent conformational changes of bovine Cu , Zn superoxide dismutase in 20 mM phosphate buffer ( pH 7.4 ) were studied at 20 degrees C using Fourier transform infrared spectroscopy .
	manualset3
130792	4	406088	13	NULL	NULL	0	NULL	pH 7.4	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Redox-dependent conformational changes of bovine Cu , Zn superoxide dismutase in 20 mM phosphate buffer ( pH 7.4 ) were studied at 20 degrees C using Fourier transform infrared spectroscopy .
	manualset3
130793	5	406088	13	NULL	NULL	0	NULL	20 degrees C 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Redox-dependent conformational changes of bovine Cu , Zn superoxide dismutase in 20 mM phosphate buffer ( pH 7.4 ) were studied at 20 degrees C using Fourier transform infrared spectroscopy .
	manualset3
130794	6	406088	13	NULL	NULL	0	NULL	Fourier transform infrared spectroscopy 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Redox-dependent conformational changes of bovine Cu , Zn superoxide dismutase in 20 mM phosphate buffer ( pH 7.4 ) were studied at 20 degrees C using Fourier transform infrared spectroscopy .
	manualset3
130795	1	406089	13	NULL	NULL	0	NULL	Redox regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Redox regulation of Fcgamma receptor-mediated phagocytosis : implications for host defense and tissue injury .
	manualset3
130796	2	406089	13	NULL	NULL	0	NULL	Fcgamma receptor-mediated phagocytosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Redox regulation of Fcgamma receptor-mediated phagocytosis : implications for host defense and tissue injury .
	manualset3
130797	3	406089	13	NULL	NULL	0	NULL	implications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Redox regulation of Fcgamma receptor-mediated phagocytosis : implications for host defense and tissue injury .
	manualset3
130798	4	406089	13	NULL	NULL	0	NULL	host defense	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Redox regulation of Fcgamma receptor-mediated phagocytosis : implications for host defense and tissue injury .
	manualset3
130799	5	406089	13	NULL	NULL	0	NULL	tissue injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Redox regulation of Fcgamma receptor-mediated phagocytosis : implications for host defense and tissue injury .
	manualset3
130800	1	406090	13	NULL	NULL	0	NULL	Redox regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Redox regulation of angiotensin II signaling in the heart .
	manualset3
130801	2	406090	13	NULL	NULL	0	NULL	angiotensin II signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Redox regulation of angiotensin II signaling in the heart .
	manualset3
130802	3	406090	13	NULL	NULL	0	NULL	heart	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Redox regulation of angiotensin II signaling in the heart .
	manualset3
130803	1	406091	13	NULL	NULL	0	NULL	Reduced Q-0	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced Q-0 has no effect on the histidine kinases .
	manualset3
130804	2	406091	13	NULL	NULL	0	NULL	effect 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced Q-0 has no effect on the histidine kinases .
	manualset3
130805	3	406091	13	NULL	NULL	0	NULL	histidine kinases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced Q-0 has no effect on the histidine kinases .
	manualset3
130806	1	406092	13	NULL	NULL	0	NULL	erythrocyte parameters 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced erythrocyte parameters suggest that chronic feeding of the purified diet might result in anemia .
	manualset3
130807	2	406092	13	NULL	NULL	0	NULL	chronic feeding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced erythrocyte parameters suggest that chronic feeding of the purified diet might result in anemia .
	manualset3
130808	3	406092	13	NULL	NULL	0	NULL	diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced erythrocyte parameters suggest that chronic feeding of the purified diet might result in anemia .
	manualset3
130809	4	406092	13	NULL	NULL	0	NULL	anemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced erythrocyte parameters suggest that chronic feeding of the purified diet might result in anemia .
	manualset3
130810	1	406093	13	NULL	NULL	0	NULL	feed intake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced feed intake results in a diminishment of bile production and induces accumulation of e.g. PAH-metabolites in bile .
	manualset3
130812	3	406093	13	NULL	NULL	0	NULL	diminishment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced feed intake results in a diminishment of bile production and induces accumulation of e.g. PAH-metabolites in bile .
	manualset3
130813	4	406093	13	NULL	NULL	0	NULL	bile production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced feed intake results in a diminishment of bile production and induces accumulation of e.g. PAH-metabolites in bile .
	manualset3
130814	5	406093	13	NULL	NULL	0	NULL	accumulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced feed intake results in a diminishment of bile production and induces accumulation of e.g. PAH-metabolites in bile .
	manualset3
130815	6	406093	13	NULL	NULL	0	NULL	PAH-metabolites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced feed intake results in a diminishment of bile production and induces accumulation of e.g. PAH-metabolites in bile .
	manualset3
130816	7	406093	13	NULL	NULL	0	NULL	bile	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced feed intake results in a diminishment of bile production and induces accumulation of e.g. PAH-metabolites in bile .
	manualset3
130817	1	406094	13	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A model for the replication of the chloroplast DNA is based on these results .
	manualset3
130818	2	406094	13	NULL	NULL	0	NULL	replication	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A model for the replication of the chloroplast DNA is based on these results .
	manualset3
130819	3	406094	13	NULL	NULL	0	NULL	chloroplast DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A model for the replication of the chloroplast DNA is based on these results .
	manualset3
130820	4	406094	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A model for the replication of the chloroplast DNA is based on these results .
	manualset3
130821	1	406095	13	NULL	NULL	0	NULL	mortality risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced late mortality risk contributes to similar survival after double-unit cord blood transplantation compared with related and unrelated donor hematopoietic stem cell transplantation .
	manualset3
130822	2	406095	13	NULL	NULL	0	NULL	survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced late mortality risk contributes to similar survival after double-unit cord blood transplantation compared with related and unrelated donor hematopoietic stem cell transplantation .
	manualset3
130823	3	406095	13	NULL	NULL	0	NULL	double-unit cord blood transplantation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced late mortality risk contributes to similar survival after double-unit cord blood transplantation compared with related and unrelated donor hematopoietic stem cell transplantation .
	manualset3
130824	4	406095	13	NULL	NULL	0	NULL	related hematopoietic stem cell transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced late mortality risk contributes to similar survival after double-unit cord blood transplantation compared with related and unrelated donor hematopoietic stem cell transplantation .
	manualset3
130825	5	406095	13	NULL	NULL	0	NULL	unrelated donor hematopoietic stem cell transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced late mortality risk contributes to similar survival after double-unit cord blood transplantation compared with related and unrelated donor hematopoietic stem cell transplantation .
	manualset3
130826	1	406096	13	NULL	NULL	0	NULL	rat erythrocyte lifetimes	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced rat erythrocyte lifetimes and elevated activities of membrane adenylate cyclase and protein kinase after glucosulfone treatment ( proceedings ) .
	manualset3
130827	2	406096	13	NULL	NULL	0	NULL	activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced rat erythrocyte lifetimes and elevated activities of membrane adenylate cyclase and protein kinase after glucosulfone treatment ( proceedings ) .
	manualset3
130828	3	406096	13	NULL	NULL	0	NULL	membrane adenylate cyclase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced rat erythrocyte lifetimes and elevated activities of membrane adenylate cyclase and protein kinase after glucosulfone treatment ( proceedings ) .
	manualset3
130829	4	406096	13	NULL	NULL	0	NULL	protein kinase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced rat erythrocyte lifetimes and elevated activities of membrane adenylate cyclase and protein kinase after glucosulfone treatment ( proceedings ) .
	manualset3
130830	5	406096	13	NULL	NULL	0	NULL	glucosulfone treatment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced rat erythrocyte lifetimes and elevated activities of membrane adenylate cyclase and protein kinase after glucosulfone treatment ( proceedings ) .
	manualset3
130831	6	406096	13	NULL	NULL	0	NULL	proceedings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced rat erythrocyte lifetimes and elevated activities of membrane adenylate cyclase and protein kinase after glucosulfone treatment ( proceedings ) .
	manualset3
130832	1	406097	13	NULL	NULL	0	NULL	stretch reflex sensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced stretch reflex sensitivity and muscle stiffness after long-lasting stretch-shortening cycle exercise in humans .
	manualset3
130833	2	406097	13	NULL	NULL	0	NULL	muscle stiffness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced stretch reflex sensitivity and muscle stiffness after long-lasting stretch-shortening cycle exercise in humans .
	manualset3
130834	3	406097	13	NULL	NULL	0	NULL	cycle exercise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced stretch reflex sensitivity and muscle stiffness after long-lasting stretch-shortening cycle exercise in humans .
	manualset3
130835	4	406097	13	NULL	NULL	0	NULL	humans 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced stretch reflex sensitivity and muscle stiffness after long-lasting stretch-shortening cycle exercise in humans .
	manualset3
130836	1	406098	13	NULL	NULL	0	NULL	Reduction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduction of inflammatory response in the mouse brain with adenoviral-mediated transforming growth factor-ss1 expression .
	manualset3
130837	2	406098	13	NULL	NULL	0	NULL	inflammatory response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduction of inflammatory response in the mouse brain with adenoviral-mediated transforming growth factor-ss1 expression .
	manualset3
130838	3	406098	13	NULL	NULL	0	NULL	mouse brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduction of inflammatory response in the mouse brain with adenoviral-mediated transforming growth factor-ss1 expression .
	manualset3
130839	4	406098	13	NULL	NULL	0	NULL	adenoviral-mediated transforming growth factor-ss1 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduction of inflammatory response in the mouse brain with adenoviral-mediated transforming growth factor-ss1 expression .
	manualset3
130840	1	406099	13	NULL	NULL	0	NULL	Reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduction of pH0 from 7.4 to 6.4 reversibly reduced pH1 by about 0.4 pH units , independent of the buffer system used .
	manualset3
130841	2	406099	13	NULL	NULL	0	NULL	pH0	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduction of pH0 from 7.4 to 6.4 reversibly reduced pH1 by about 0.4 pH units , independent of the buffer system used .
	manualset3
130842	3	406099	13	NULL	NULL	0	NULL	7.4 to 6.4	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduction of pH0 from 7.4 to 6.4 reversibly reduced pH1 by about 0.4 pH units , independent of the buffer system used .
	manualset3
130843	4	406099	13	NULL	NULL	0	NULL	pH1	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduction of pH0 from 7.4 to 6.4 reversibly reduced pH1 by about 0.4 pH units , independent of the buffer system used .
	manualset3
130844	5	406099	13	NULL	NULL	0	NULL	 0.4 pH units	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduction of pH0 from 7.4 to 6.4 reversibly reduced pH1 by about 0.4 pH units , independent of the buffer system used .
	manualset3
130845	6	406099	13	NULL	NULL	0	NULL	buffer system	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduction of pH0 from 7.4 to 6.4 reversibly reduced pH1 by about 0.4 pH units , independent of the buffer system used .
	manualset3
130846	1	406100	13	NULL	NULL	0	NULL	Reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduction of the - catenin levels in acute myeloid leukemia ( AML ) cell lines and patient samples decelerated their in vitro proliferation ability without affecting cell viability .
	manualset3
130847	2	406100	13	NULL	NULL	0	NULL	catenin levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduction of the - catenin levels in acute myeloid leukemia ( AML ) cell lines and patient samples decelerated their in vitro proliferation ability without affecting cell viability .
	manualset3
130848	3	406100	13	NULL	NULL	0	NULL	acute myeloid leukemia ( AML ) cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduction of the - catenin levels in acute myeloid leukemia ( AML ) cell lines and patient samples decelerated their in vitro proliferation ability without affecting cell viability .
	manualset3
130849	4	406100	13	NULL	NULL	NULL	NULL	patient samples 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Reduction of the - catenin levels in acute myeloid leukemia ( AML ) cell lines and patient samples decelerated their in vitro proliferation ability without affecting cell viability .
	manualset3
130850	5	406100	13	NULL	NULL	0	NULL	proliferation ability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduction of the - catenin levels in acute myeloid leukemia ( AML ) cell lines and patient samples decelerated their in vitro proliferation ability without affecting cell viability .
	manualset3
130851	6	406100	13	NULL	NULL	0	NULL	cell viability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduction of the - catenin levels in acute myeloid leukemia ( AML ) cell lines and patient samples decelerated their in vitro proliferation ability without affecting cell viability .
	manualset3
130852	1	406101	13	NULL	NULL	0	NULL	Reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduction of the dose of beclomethasone from 400 microgram/day caused worsening of asthma .
	manualset3
130853	2	406101	13	NULL	NULL	0	NULL	dose 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduction of the dose of beclomethasone from 400 microgram/day caused worsening of asthma .
	manualset3
130854	3	406101	13	NULL	NULL	0	NULL	beclomethasone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduction of the dose of beclomethasone from 400 microgram/day caused worsening of asthma .
	manualset3
130855	4	406101	13	NULL	NULL	0	NULL	 400 microgram/day 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduction of the dose of beclomethasone from 400 microgram/day caused worsening of asthma .
	manualset3
130856	5	406101	13	NULL	NULL	0	NULL	asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduction of the dose of beclomethasone from 400 microgram/day caused worsening of asthma .
	manualset3
130857	1	406102	13	NULL	NULL	0	NULL	Reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduction of visceral adipose tissue and improvement of metabolic indices : effect of dexfenfluramine in NIDDM .
	manualset3
130858	2	406102	13	NULL	NULL	0	NULL	visceral adipose tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduction of visceral adipose tissue and improvement of metabolic indices : effect of dexfenfluramine in NIDDM .
	manualset3
130859	3	406102	13	NULL	NULL	0	NULL	improvement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduction of visceral adipose tissue and improvement of metabolic indices : effect of dexfenfluramine in NIDDM .
	manualset3
130860	4	406102	13	NULL	NULL	0	NULL	metabolic indices	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduction of visceral adipose tissue and improvement of metabolic indices : effect of dexfenfluramine in NIDDM .
	manualset3
130861	5	406102	13	NULL	NULL	0	NULL	effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduction of visceral adipose tissue and improvement of metabolic indices : effect of dexfenfluramine in NIDDM .
	manualset3
130862	6	406102	13	NULL	NULL	0	NULL	dexfenfluramine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduction of visceral adipose tissue and improvement of metabolic indices : effect of dexfenfluramine in NIDDM .
	manualset3
130863	7	406102	13	NULL	NULL	0	NULL	NIDDM	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduction of visceral adipose tissue and improvement of metabolic indices : effect of dexfenfluramine in NIDDM .
	manualset3
130864	1	406103	13	NULL	NULL	0	NULL	Reductions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reductions in the incidence and severity of somatic symptoms associated with the menstrual cycle were also observed , suggesting a beneficial effect due to the antimineralocorticoid nature of drospirenone .
	manualset3
130865	2	406103	13	NULL	NULL	0	NULL	incidence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reductions in the incidence and severity of somatic symptoms associated with the menstrual cycle were also observed , suggesting a beneficial effect due to the antimineralocorticoid nature of drospirenone .
	manualset3
130866	3	406103	13	NULL	NULL	0	NULL	severity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reductions in the incidence and severity of somatic symptoms associated with the menstrual cycle were also observed , suggesting a beneficial effect due to the antimineralocorticoid nature of drospirenone .
	manualset3
130867	4	406103	13	NULL	NULL	0	NULL	somatic symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reductions in the incidence and severity of somatic symptoms associated with the menstrual cycle were also observed , suggesting a beneficial effect due to the antimineralocorticoid nature of drospirenone .
	manualset3
130868	5	406103	13	NULL	NULL	0	NULL	menstrual cycle	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reductions in the incidence and severity of somatic symptoms associated with the menstrual cycle were also observed , suggesting a beneficial effect due to the antimineralocorticoid nature of drospirenone .
	manualset3
130869	6	406103	13	NULL	NULL	0	NULL	beneficial effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reductions in the incidence and severity of somatic symptoms associated with the menstrual cycle were also observed , suggesting a beneficial effect due to the antimineralocorticoid nature of drospirenone .
	manualset3
130870	7	406103	13	NULL	NULL	0	NULL	antimineralocorticoid nature 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reductions in the incidence and severity of somatic symptoms associated with the menstrual cycle were also observed , suggesting a beneficial effect due to the antimineralocorticoid nature of drospirenone .
	manualset3
130871	8	406103	13	NULL	NULL	0	NULL	drospirenone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Reductions in the incidence and severity of somatic symptoms associated with the menstrual cycle were also observed , suggesting a beneficial effect due to the antimineralocorticoid nature of drospirenone .
	manualset3
130872	1	406104	13	NULL	NULL	0	NULL	Reductive addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reductive addition of glutathione to p-benzoquinone , 2-hydroxy-p-benzoquinone , and p-benzoquinone epoxides .
	manualset3
130873	2	406104	13	NULL	NULL	0	NULL	glutathione to p-benzoquinone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Reductive addition of glutathione to p-benzoquinone , 2-hydroxy-p-benzoquinone , and p-benzoquinone epoxides .
	manualset3
130874	3	406104	13	NULL	NULL	0	NULL	 2-hydroxy-p-benzoquinone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Reductive addition of glutathione to p-benzoquinone , 2-hydroxy-p-benzoquinone , and p-benzoquinone epoxides .
	manualset3
130875	4	406104	13	NULL	NULL	0	NULL	p-benzoquinone epoxides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Reductive addition of glutathione to p-benzoquinone , 2-hydroxy-p-benzoquinone , and p-benzoquinone epoxides .
	manualset3
130876	1	406105	13	NULL	NULL	0	NULL	Redundant spin coupling pathways	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Redundant spin coupling pathways provide ways of resolving overlaps frequently encountered in homonuclear 1H 2D NMR spectra and facilitate the elucidation of complex proton spin systems .
	manualset3
130877	2	406105	13	NULL	NULL	0	NULL	ways	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Redundant spin coupling pathways provide ways of resolving overlaps frequently encountered in homonuclear 1H 2D NMR spectra and facilitate the elucidation of complex proton spin systems .
	manualset3
130878	3	406105	13	NULL	NULL	0	NULL	homonuclear 1H 2D NMR spectra	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Redundant spin coupling pathways provide ways of resolving overlaps frequently encountered in homonuclear 1H 2D NMR spectra and facilitate the elucidation of complex proton spin systems .
	manualset3
130879	4	406105	13	NULL	NULL	0	NULL	elucidation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Redundant spin coupling pathways provide ways of resolving overlaps frequently encountered in homonuclear 1H 2D NMR spectra and facilitate the elucidation of complex proton spin systems .
	manualset3
130880	5	406105	13	NULL	NULL	0	NULL	complex proton spin systems	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Redundant spin coupling pathways provide ways of resolving overlaps frequently encountered in homonuclear 1H 2D NMR spectra and facilitate the elucidation of complex proton spin systems .
	manualset3
130882	2	406106	13	NULL	NULL	0	NULL	drug plan reimbursement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reference pricing ( RP ) limits drug plan reimbursement of interchangeable medicines to a reference price , which is typically equal to the price of the lowest-cost interchangeable drug ; any cost above that is borne by the patient .
	manualset3
130883	3	406106	13	NULL	NULL	0	NULL	interchangeable medicines	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Reference pricing ( RP ) limits drug plan reimbursement of interchangeable medicines to a reference price , which is typically equal to the price of the lowest-cost interchangeable drug ; any cost above that is borne by the patient .
	manualset3
130884	4	406106	13	NULL	NULL	NULL	NULL	Reference pricing ( RP ) 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Reference pricing ( RP ) limits drug plan reimbursement of interchangeable medicines to a reference price , which is typically equal to the price of the lowest-cost interchangeable drug ; any cost above that is borne by the patient .
	manualset3
130885	5	406106	13	NULL	NULL	0	NULL	price	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Reference pricing ( RP ) limits drug plan reimbursement of interchangeable medicines to a reference price , which is typically equal to the price of the lowest-cost interchangeable drug ; any cost above that is borne by the patient .
	manualset3
130886	6	406106	13	NULL	NULL	0	NULL	lowest-cost interchangeable drug 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Reference pricing ( RP ) limits drug plan reimbursement of interchangeable medicines to a reference price , which is typically equal to the price of the lowest-cost interchangeable drug ; any cost above that is borne by the patient .
	manualset3
130887	7	406106	13	NULL	NULL	0	NULL	cost 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Reference pricing ( RP ) limits drug plan reimbursement of interchangeable medicines to a reference price , which is typically equal to the price of the lowest-cost interchangeable drug ; any cost above that is borne by the patient .
	manualset3
130888	8	406106	13	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Reference pricing ( RP ) limits drug plan reimbursement of interchangeable medicines to a reference price , which is typically equal to the price of the lowest-cost interchangeable drug ; any cost above that is borne by the patient .
	manualset3
130889	1	406107	13	NULL	NULL	0	NULL	Carcinomatous degeneration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Carcinomatous degeneration in lesions of erythematodes ) .
	manualset3
130890	2	406107	13	NULL	NULL	0	NULL	 lesions of erythematodes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Carcinomatous degeneration in lesions of erythematodes ) .
	manualset3
130891	1	406108	13	NULL	NULL	0	NULL	model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A model of biological motion perception from configural form cues .
	manualset3
130892	2	406108	13	NULL	NULL	0	NULL	biological motion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A model of biological motion perception from configural form cues .
	manualset3
130893	3	406108	13	NULL	NULL	0	NULL	perception 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A model of biological motion perception from configural form cues .
	manualset3
130894	4	406108	13	NULL	NULL	0	NULL	configural form cues 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A model of biological motion perception from configural form cues .
	manualset3
130895	1	406109	13	NULL	NULL	0	NULL	physical mapping	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Refined physical mapping and genomic structure of the EXTL1 gene .
	manualset3
130896	2	406109	13	NULL	NULL	0	NULL	genomic structure 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Refined physical mapping and genomic structure of the EXTL1 gene .
	manualset3
130897	3	406109	13	NULL	NULL	0	NULL	EXTL1 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Refined physical mapping and genomic structure of the EXTL1 gene .
	manualset3
130898	1	406110	13	NULL	NULL	0	NULL	Refinement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Refinement of the locus for autosomal dominant juvenile optic atrophy to a 2 cM region on 3q28 .
	manualset3
130899	2	406110	13	NULL	NULL	0	NULL	locus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Refinement of the locus for autosomal dominant juvenile optic atrophy to a 2 cM region on 3q28 .
	manualset3
130900	3	406110	13	NULL	NULL	0	NULL	 autosomal dominant juvenile optic atrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Refinement of the locus for autosomal dominant juvenile optic atrophy to a 2 cM region on 3q28 .
	manualset3
130901	4	406110	13	NULL	NULL	0	NULL	2 cM region 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Refinement of the locus for autosomal dominant juvenile optic atrophy to a 2 cM region on 3q28 .
	manualset3
130902	5	406110	13	NULL	NULL	0	NULL	3q28	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Refinement of the locus for autosomal dominant juvenile optic atrophy to a 2 cM region on 3q28 .
	manualset3
130903	1	406111	13	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Refining the relationship between homozygosity and the frequency of the most frequent allele .
	manualset3
130904	2	406111	13	NULL	NULL	0	NULL	homozygosity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Refining the relationship between homozygosity and the frequency of the most frequent allele .
	manualset3
130905	3	406111	13	NULL	NULL	0	NULL	frequency	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Refining the relationship between homozygosity and the frequency of the most frequent allele .
	manualset3
130906	4	406111	13	NULL	NULL	0	NULL	allele	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Refining the relationship between homozygosity and the frequency of the most frequent allele .
	manualset3
130907	1	406112	13	NULL	NULL	0	NULL	Refixation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Refixation of the scleral flap into its bed with sutures is an essential feature of the operation .
	manualset3
130908	2	406112	13	NULL	NULL	0	NULL	scleral flap	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Refixation of the scleral flap into its bed with sutures is an essential feature of the operation .
	manualset3
130909	3	406112	13	NULL	NULL	0	NULL	bed	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Refixation of the scleral flap into its bed with sutures is an essential feature of the operation .
	manualset3
130910	4	406112	13	NULL	NULL	0	NULL	sutures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Refixation of the scleral flap into its bed with sutures is an essential feature of the operation .
	manualset3
130911	5	406112	13	NULL	NULL	0	NULL	essential feature	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Refixation of the scleral flap into its bed with sutures is an essential feature of the operation .
	manualset3
130912	6	406112	13	NULL	NULL	0	NULL	operation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Refixation of the scleral flap into its bed with sutures is an essential feature of the operation .
	manualset3
130913	1	406113	13	NULL	NULL	0	NULL	Reflections	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reflections on a bone marrow transplant .
	manualset3
130914	2	406113	13	NULL	NULL	0	NULL	bone marrow transplant	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Reflections on a bone marrow transplant .
	manualset3
130916	2	406114	13	NULL	NULL	0	NULL	autobiographical accounts	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Reflective and insightful autobiographical accounts of illness not only illuminate fundamental disruptions in selfhood and continuity of life that accompany illness , but authors of such accounts also maintain that narration is an important way to make sense of an illness episode , to restore personhood and connectedness , and to reclaim the illness experience from the medical meta-narrative .
	manualset3
130917	3	406114	13	NULL	NULL	0	NULL	illness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reflective and insightful autobiographical accounts of illness not only illuminate fundamental disruptions in selfhood and continuity of life that accompany illness , but authors of such accounts also maintain that narration is an important way to make sense of an illness episode , to restore personhood and connectedness , and to reclaim the illness experience from the medical meta-narrative .
	manualset3
130918	4	406114	13	NULL	NULL	0	NULL	disruptions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reflective and insightful autobiographical accounts of illness not only illuminate fundamental disruptions in selfhood and continuity of life that accompany illness , but authors of such accounts also maintain that narration is an important way to make sense of an illness episode , to restore personhood and connectedness , and to reclaim the illness experience from the medical meta-narrative .
	manualset3
130919	5	406114	13	NULL	NULL	0	NULL	selfhood 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reflective and insightful autobiographical accounts of illness not only illuminate fundamental disruptions in selfhood and continuity of life that accompany illness , but authors of such accounts also maintain that narration is an important way to make sense of an illness episode , to restore personhood and connectedness , and to reclaim the illness experience from the medical meta-narrative .
	manualset3
130920	6	406114	13	NULL	NULL	0	NULL	continuity of life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reflective and insightful autobiographical accounts of illness not only illuminate fundamental disruptions in selfhood and continuity of life that accompany illness , but authors of such accounts also maintain that narration is an important way to make sense of an illness episode , to restore personhood and connectedness , and to reclaim the illness experience from the medical meta-narrative .
	manualset3
130921	7	406114	13	NULL	NULL	0	NULL	illness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reflective and insightful autobiographical accounts of illness not only illuminate fundamental disruptions in selfhood and continuity of life that accompany illness , but authors of such accounts also maintain that narration is an important way to make sense of an illness episode , to restore personhood and connectedness , and to reclaim the illness experience from the medical meta-narrative .
	manualset3
130922	8	406114	13	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Reflective and insightful autobiographical accounts of illness not only illuminate fundamental disruptions in selfhood and continuity of life that accompany illness , but authors of such accounts also maintain that narration is an important way to make sense of an illness episode , to restore personhood and connectedness , and to reclaim the illness experience from the medical meta-narrative .
	manualset3
130923	9	406114	13	NULL	NULL	0	NULL	accounts	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Reflective and insightful autobiographical accounts of illness not only illuminate fundamental disruptions in selfhood and continuity of life that accompany illness , but authors of such accounts also maintain that narration is an important way to make sense of an illness episode , to restore personhood and connectedness , and to reclaim the illness experience from the medical meta-narrative .
	manualset3
130924	10	406114	13	NULL	NULL	0	NULL	narration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reflective and insightful autobiographical accounts of illness not only illuminate fundamental disruptions in selfhood and continuity of life that accompany illness , but authors of such accounts also maintain that narration is an important way to make sense of an illness episode , to restore personhood and connectedness , and to reclaim the illness experience from the medical meta-narrative .
	manualset3
130925	11	406114	13	NULL	NULL	0	NULL	way 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reflective and insightful autobiographical accounts of illness not only illuminate fundamental disruptions in selfhood and continuity of life that accompany illness , but authors of such accounts also maintain that narration is an important way to make sense of an illness episode , to restore personhood and connectedness , and to reclaim the illness experience from the medical meta-narrative .
	manualset3
130926	12	406114	13	NULL	NULL	0	NULL	illness episode	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reflective and insightful autobiographical accounts of illness not only illuminate fundamental disruptions in selfhood and continuity of life that accompany illness , but authors of such accounts also maintain that narration is an important way to make sense of an illness episode , to restore personhood and connectedness , and to reclaim the illness experience from the medical meta-narrative .
	manualset3
130927	13	406114	13	NULL	NULL	0	NULL	personhood 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reflective and insightful autobiographical accounts of illness not only illuminate fundamental disruptions in selfhood and continuity of life that accompany illness , but authors of such accounts also maintain that narration is an important way to make sense of an illness episode , to restore personhood and connectedness , and to reclaim the illness experience from the medical meta-narrative .
	manualset3
130928	14	406114	13	NULL	NULL	0	NULL	connectedness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reflective and insightful autobiographical accounts of illness not only illuminate fundamental disruptions in selfhood and continuity of life that accompany illness , but authors of such accounts also maintain that narration is an important way to make sense of an illness episode , to restore personhood and connectedness , and to reclaim the illness experience from the medical meta-narrative .
	manualset3
130929	15	406114	13	NULL	NULL	0	NULL	illness experience	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reflective and insightful autobiographical accounts of illness not only illuminate fundamental disruptions in selfhood and continuity of life that accompany illness , but authors of such accounts also maintain that narration is an important way to make sense of an illness episode , to restore personhood and connectedness , and to reclaim the illness experience from the medical meta-narrative .
	manualset3
130930	16	406114	13	NULL	NULL	0	NULL	medical meta-narrative	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reflective and insightful autobiographical accounts of illness not only illuminate fundamental disruptions in selfhood and continuity of life that accompany illness , but authors of such accounts also maintain that narration is an important way to make sense of an illness episode , to restore personhood and connectedness , and to reclaim the illness experience from the medical meta-narrative .
	manualset3
130931	1	406115	13	NULL	NULL	0	NULL	Reflex forearm vasoconstriction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reflex forearm vasoconstriction in response to lower body negative pressure at 40 mm Hg was less in the early convalescent phase ( mean seven days ) than in the late convalescent phase ( mean 41 days ) .
	manualset3
130932	2	406115	13	NULL	NULL	0	NULL	response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reflex forearm vasoconstriction in response to lower body negative pressure at 40 mm Hg was less in the early convalescent phase ( mean seven days ) than in the late convalescent phase ( mean 41 days ) .
	manualset3
130933	3	406115	13	NULL	NULL	0	NULL	lower body negative pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reflex forearm vasoconstriction in response to lower body negative pressure at 40 mm Hg was less in the early convalescent phase ( mean seven days ) than in the late convalescent phase ( mean 41 days ) .
	manualset3
130934	4	406115	13	NULL	NULL	0	NULL	40 mm Hg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Reflex forearm vasoconstriction in response to lower body negative pressure at 40 mm Hg was less in the early convalescent phase ( mean seven days ) than in the late convalescent phase ( mean 41 days ) .
	manualset3
130935	5	406115	13	NULL	NULL	NULL	NULL	early convalescent phase 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Reflex forearm vasoconstriction in response to lower body negative pressure at 40 mm Hg was less in the early convalescent phase ( mean seven days ) than in the late convalescent phase ( mean 41 days ) .
	manualset3
130936	6	406115	13	NULL	NULL	0	NULL	mean seven days	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Reflex forearm vasoconstriction in response to lower body negative pressure at 40 mm Hg was less in the early convalescent phase ( mean seven days ) than in the late convalescent phase ( mean 41 days ) .
	manualset3
130937	7	406115	13	NULL	NULL	0	NULL	late convalescent phase	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Reflex forearm vasoconstriction in response to lower body negative pressure at 40 mm Hg was less in the early convalescent phase ( mean seven days ) than in the late convalescent phase ( mean 41 days ) .
	manualset3
130938	8	406115	13	NULL	NULL	NULL	NULL	mean 41 days	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Reflex forearm vasoconstriction in response to lower body negative pressure at 40 mm Hg was less in the early convalescent phase ( mean seven days ) than in the late convalescent phase ( mean 41 days ) .
	manualset3
130939	1	406116	13	NULL	NULL	0	NULL	barriers	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding barriers , 15 % reported that the physician had never requested it , 10.9 % did not consider it important and 16.9 % were afraid to take the examination .
	manualset3
130940	2	406116	13	NULL	NULL	0	NULL	15 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding barriers , 15 % reported that the physician had never requested it , 10.9 % did not consider it important and 16.9 % were afraid to take the examination .
	manualset3
130941	3	406116	13	NULL	NULL	0	NULL	physician	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding barriers , 15 % reported that the physician had never requested it , 10.9 % did not consider it important and 16.9 % were afraid to take the examination .
	manualset3
130942	4	406116	13	NULL	NULL	0	NULL	10.9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding barriers , 15 % reported that the physician had never requested it , 10.9 % did not consider it important and 16.9 % were afraid to take the examination .
	manualset3
130943	5	406116	13	NULL	NULL	0	NULL	16.9 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding barriers , 15 % reported that the physician had never requested it , 10.9 % did not consider it important and 16.9 % were afraid to take the examination .
	manualset3
130944	6	406116	13	NULL	NULL	0	NULL	examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding barriers , 15 % reported that the physician had never requested it , 10.9 % did not consider it important and 16.9 % were afraid to take the examination .
	manualset3
130945	1	406117	13	NULL	NULL	0	NULL	details of epidemiology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding details of epidemiology , pathogenesis , diagnosis and prevention of ETEC infections and diarrhoea in animals , readers are referred to an earlier more extensive review ( Nagy and Fekete , 1999 .
	manualset3
130946	2	406117	13	NULL	NULL	0	NULL	pathogenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding details of epidemiology , pathogenesis , diagnosis and prevention of ETEC infections and diarrhoea in animals , readers are referred to an earlier more extensive review ( Nagy and Fekete , 1999 .
	manualset3
130947	3	406117	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding details of epidemiology , pathogenesis , diagnosis and prevention of ETEC infections and diarrhoea in animals , readers are referred to an earlier more extensive review ( Nagy and Fekete , 1999 .
	manualset3
130948	4	406117	13	NULL	NULL	0	NULL	prevention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding details of epidemiology , pathogenesis , diagnosis and prevention of ETEC infections and diarrhoea in animals , readers are referred to an earlier more extensive review ( Nagy and Fekete , 1999 .
	manualset3
130949	5	406117	13	NULL	NULL	0	NULL	ETEC infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding details of epidemiology , pathogenesis , diagnosis and prevention of ETEC infections and diarrhoea in animals , readers are referred to an earlier more extensive review ( Nagy and Fekete , 1999 .
	manualset3
130950	6	406117	13	NULL	NULL	0	NULL	diarrhoea	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding details of epidemiology , pathogenesis , diagnosis and prevention of ETEC infections and diarrhoea in animals , readers are referred to an earlier more extensive review ( Nagy and Fekete , 1999 .
	manualset3
130951	7	406117	13	NULL	NULL	0	NULL	animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding details of epidemiology , pathogenesis , diagnosis and prevention of ETEC infections and diarrhoea in animals , readers are referred to an earlier more extensive review ( Nagy and Fekete , 1999 .
	manualset3
130952	8	406117	13	NULL	NULL	0	NULL	readers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding details of epidemiology , pathogenesis , diagnosis and prevention of ETEC infections and diarrhoea in animals , readers are referred to an earlier more extensive review ( Nagy and Fekete , 1999 .
	manualset3
130953	9	406117	13	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding details of epidemiology , pathogenesis , diagnosis and prevention of ETEC infections and diarrhoea in animals , readers are referred to an earlier more extensive review ( Nagy and Fekete , 1999 .
	manualset3
130954	10	406117	13	NULL	NULL	0	NULL	Nagy	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding details of epidemiology , pathogenesis , diagnosis and prevention of ETEC infections and diarrhoea in animals , readers are referred to an earlier more extensive review ( Nagy and Fekete , 1999 .
	manualset3
130955	11	406117	13	NULL	NULL	0	NULL	Fekete	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding details of epidemiology , pathogenesis , diagnosis and prevention of ETEC infections and diarrhoea in animals , readers are referred to an earlier more extensive review ( Nagy and Fekete , 1999 .
	manualset3
130956	12	406117	13	NULL	NULL	0	NULL	1999	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding details of epidemiology , pathogenesis , diagnosis and prevention of ETEC infections and diarrhoea in animals , readers are referred to an earlier more extensive review ( Nagy and Fekete , 1999 .
	manualset3
130957	1	406118	13	NULL	NULL	0	NULL	item memory 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding item memory , adults showed the putative ERP correlates of familiarity and recollection , whereas ERP effects in children and adolescents suggested a strong reliance on recollection .
	manualset3
130958	2	406118	13	NULL	NULL	0	NULL	adults 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding item memory , adults showed the putative ERP correlates of familiarity and recollection , whereas ERP effects in children and adolescents suggested a strong reliance on recollection .
	manualset3
130959	3	406118	13	NULL	NULL	0	NULL	putative ERP	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding item memory , adults showed the putative ERP correlates of familiarity and recollection , whereas ERP effects in children and adolescents suggested a strong reliance on recollection .
	manualset3
130960	4	406118	13	NULL	NULL	0	NULL	familiarity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding item memory , adults showed the putative ERP correlates of familiarity and recollection , whereas ERP effects in children and adolescents suggested a strong reliance on recollection .
	manualset3
130961	5	406118	13	NULL	NULL	0	NULL	recollection 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding item memory , adults showed the putative ERP correlates of familiarity and recollection , whereas ERP effects in children and adolescents suggested a strong reliance on recollection .
	manualset3
130962	6	406118	13	NULL	NULL	0	NULL	ERP effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding item memory , adults showed the putative ERP correlates of familiarity and recollection , whereas ERP effects in children and adolescents suggested a strong reliance on recollection .
	manualset3
130963	7	406118	13	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding item memory , adults showed the putative ERP correlates of familiarity and recollection , whereas ERP effects in children and adolescents suggested a strong reliance on recollection .
	manualset3
130964	8	406118	13	NULL	NULL	0	NULL	adolescents 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding item memory , adults showed the putative ERP correlates of familiarity and recollection , whereas ERP effects in children and adolescents suggested a strong reliance on recollection .
	manualset3
130965	9	406118	13	NULL	NULL	0	NULL	reliance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding item memory , adults showed the putative ERP correlates of familiarity and recollection , whereas ERP effects in children and adolescents suggested a strong reliance on recollection .
	manualset3
130966	10	406118	13	NULL	NULL	0	NULL	recollection	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding item memory , adults showed the putative ERP correlates of familiarity and recollection , whereas ERP effects in children and adolescents suggested a strong reliance on recollection .
	manualset3
130967	1	406119	13	NULL	NULL	0	NULL	selectivity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding selectivity , the receptor showed stereoselective binding toward those substrates bearing an H-bonding donor at Calpha , being S-selective in most of the cases , except for glutamic acid .
	manualset3
130968	2	406119	13	NULL	NULL	0	NULL	receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding selectivity , the receptor showed stereoselective binding toward those substrates bearing an H-bonding donor at Calpha , being S-selective in most of the cases , except for glutamic acid .
	manualset3
130969	3	406119	13	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding selectivity , the receptor showed stereoselective binding toward those substrates bearing an H-bonding donor at Calpha , being S-selective in most of the cases , except for glutamic acid .
	manualset3
130970	4	406119	13	NULL	NULL	NULL	NULL	substrates	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Regarding selectivity , the receptor showed stereoselective binding toward those substrates bearing an H-bonding donor at Calpha , being S-selective in most of the cases , except for glutamic acid .
	manualset3
130971	5	406119	13	NULL	NULL	0	NULL	H-bonding donor at Calpha	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding selectivity , the receptor showed stereoselective binding toward those substrates bearing an H-bonding donor at Calpha , being S-selective in most of the cases , except for glutamic acid .
	manualset3
130972	6	406119	13	NULL	NULL	0	NULL	cases	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding selectivity , the receptor showed stereoselective binding toward those substrates bearing an H-bonding donor at Calpha , being S-selective in most of the cases , except for glutamic acid .
	manualset3
130973	7	406119	13	NULL	NULL	0	NULL	glutamic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding selectivity , the receptor showed stereoselective binding toward those substrates bearing an H-bonding donor at Calpha , being S-selective in most of the cases , except for glutamic acid .
	manualset3
130974	1	406120	13	NULL	NULL	0	NULL	removal efficiency 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding the removal efficiency the prepared samples attained values comparable to a commercial carbon ( & gt ; 65 % ) , revealing that chemical activation of sisal wastes with K ( 2 ) CO ( 3 ) allows obtaining samples suitable for pharmaceutical compounds removal from liquid phase .
	manualset3
130975	2	406120	13	NULL	NULL	0	NULL	samples	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding the removal efficiency the prepared samples attained values comparable to a commercial carbon ( & gt ; 65 % ) , revealing that chemical activation of sisal wastes with K ( 2 ) CO ( 3 ) allows obtaining samples suitable for pharmaceutical compounds removal from liquid phase .
	manualset3
130976	3	406120	13	NULL	NULL	0	NULL	values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding the removal efficiency the prepared samples attained values comparable to a commercial carbon ( & gt ; 65 % ) , revealing that chemical activation of sisal wastes with K ( 2 ) CO ( 3 ) allows obtaining samples suitable for pharmaceutical compounds removal from liquid phase .
	manualset3
130977	4	406120	13	NULL	NULL	0	NULL	carbon	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding the removal efficiency the prepared samples attained values comparable to a commercial carbon ( & gt ; 65 % ) , revealing that chemical activation of sisal wastes with K ( 2 ) CO ( 3 ) allows obtaining samples suitable for pharmaceutical compounds removal from liquid phase .
	manualset3
130978	5	406120	13	NULL	NULL	0	NULL	65 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding the removal efficiency the prepared samples attained values comparable to a commercial carbon ( & gt ; 65 % ) , revealing that chemical activation of sisal wastes with K ( 2 ) CO ( 3 ) allows obtaining samples suitable for pharmaceutical compounds removal from liquid phase .
	manualset3
130979	6	406120	13	NULL	NULL	0	NULL	chemical activation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding the removal efficiency the prepared samples attained values comparable to a commercial carbon ( & gt ; 65 % ) , revealing that chemical activation of sisal wastes with K ( 2 ) CO ( 3 ) allows obtaining samples suitable for pharmaceutical compounds removal from liquid phase .
	manualset3
130980	7	406120	13	NULL	NULL	0	NULL	sisal wastes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding the removal efficiency the prepared samples attained values comparable to a commercial carbon ( & gt ; 65 % ) , revealing that chemical activation of sisal wastes with K ( 2 ) CO ( 3 ) allows obtaining samples suitable for pharmaceutical compounds removal from liquid phase .
	manualset3
130981	8	406120	13	NULL	NULL	0	NULL	K ( 2 ) CO ( 3 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding the removal efficiency the prepared samples attained values comparable to a commercial carbon ( & gt ; 65 % ) , revealing that chemical activation of sisal wastes with K ( 2 ) CO ( 3 ) allows obtaining samples suitable for pharmaceutical compounds removal from liquid phase .
	manualset3
130982	9	406120	13	NULL	NULL	0	NULL	samples	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding the removal efficiency the prepared samples attained values comparable to a commercial carbon ( & gt ; 65 % ) , revealing that chemical activation of sisal wastes with K ( 2 ) CO ( 3 ) allows obtaining samples suitable for pharmaceutical compounds removal from liquid phase .
	manualset3
130983	10	406120	13	NULL	NULL	0	NULL	pharmaceutical compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding the removal efficiency the prepared samples attained values comparable to a commercial carbon ( & gt ; 65 % ) , revealing that chemical activation of sisal wastes with K ( 2 ) CO ( 3 ) allows obtaining samples suitable for pharmaceutical compounds removal from liquid phase .
	manualset3
130984	11	406120	13	NULL	NULL	0	NULL	removal 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding the removal efficiency the prepared samples attained values comparable to a commercial carbon ( & gt ; 65 % ) , revealing that chemical activation of sisal wastes with K ( 2 ) CO ( 3 ) allows obtaining samples suitable for pharmaceutical compounds removal from liquid phase .
	manualset3
130985	12	406120	13	NULL	NULL	0	NULL	liquid phase	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding the removal efficiency the prepared samples attained values comparable to a commercial carbon ( & gt ; 65 % ) , revealing that chemical activation of sisal wastes with K ( 2 ) CO ( 3 ) allows obtaining samples suitable for pharmaceutical compounds removal from liquid phase .
	manualset3
130986	1	406121	13	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding the results of the workplace-based studies it could be predicted that 20 , 000 out of 220 , 000 workers in mining sector could have pneumoconiosis and approximately 5 , 000 new pneumoconiosis cases might have occurred each year .
	manualset3
130987	2	406121	13	NULL	NULL	0	NULL	workplace-based studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding the results of the workplace-based studies it could be predicted that 20 , 000 out of 220 , 000 workers in mining sector could have pneumoconiosis and approximately 5 , 000 new pneumoconiosis cases might have occurred each year .
	manualset3
130988	3	406121	13	NULL	NULL	0	NULL	20 , 000 workers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding the results of the workplace-based studies it could be predicted that 20 , 000 out of 220 , 000 workers in mining sector could have pneumoconiosis and approximately 5 , 000 new pneumoconiosis cases might have occurred each year .
	manualset3
130989	4	406121	13	NULL	NULL	0	NULL	220 , 000 workers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding the results of the workplace-based studies it could be predicted that 20 , 000 out of 220 , 000 workers in mining sector could have pneumoconiosis and approximately 5 , 000 new pneumoconiosis cases might have occurred each year .
	manualset3
130990	5	406121	13	NULL	NULL	0	NULL	mining sector	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding the results of the workplace-based studies it could be predicted that 20 , 000 out of 220 , 000 workers in mining sector could have pneumoconiosis and approximately 5 , 000 new pneumoconiosis cases might have occurred each year .
	manualset3
130991	6	406121	13	NULL	NULL	0	NULL	pneumoconiosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding the results of the workplace-based studies it could be predicted that 20 , 000 out of 220 , 000 workers in mining sector could have pneumoconiosis and approximately 5 , 000 new pneumoconiosis cases might have occurred each year .
	manualset3
130992	7	406121	13	NULL	NULL	0	NULL	approximately 5 , 000 new pneumoconiosis cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding the results of the workplace-based studies it could be predicted that 20 , 000 out of 220 , 000 workers in mining sector could have pneumoconiosis and approximately 5 , 000 new pneumoconiosis cases might have occurred each year .
	manualset3
130993	8	406121	13	NULL	NULL	0	NULL	year	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding the results of the workplace-based studies it could be predicted that 20 , 000 out of 220 , 000 workers in mining sector could have pneumoconiosis and approximately 5 , 000 new pneumoconiosis cases might have occurred each year .
	manualset3
130994	1	406122	13	NULL	NULL	0	NULL	biodegradation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding ultimate biodegradation , the addition of LAS to the batch anaerobic digesters caused a reduction on the extent of biogas production .
	manualset3
130995	2	406122	13	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding ultimate biodegradation , the addition of LAS to the batch anaerobic digesters caused a reduction on the extent of biogas production .
	manualset3
130996	3	406122	13	NULL	NULL	0	NULL	LAS	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding ultimate biodegradation , the addition of LAS to the batch anaerobic digesters caused a reduction on the extent of biogas production .
	manualset3
130997	4	406122	13	NULL	NULL	0	NULL	batch anaerobic digesters	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding ultimate biodegradation , the addition of LAS to the batch anaerobic digesters caused a reduction on the extent of biogas production .
	manualset3
130998	5	406122	13	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding ultimate biodegradation , the addition of LAS to the batch anaerobic digesters caused a reduction on the extent of biogas production .
	manualset3
130999	6	406122	13	NULL	NULL	0	NULL	biogas production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regarding ultimate biodegradation , the addition of LAS to the batch anaerobic digesters caused a reduction on the extent of biogas production .
	manualset3
131001	2	406123	13	NULL	NULL	0	NULL	D-type cyclins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of butyrate 's effect on D-type cyclins , downregulation of G1-specific cdks and upregulation of cdk inhibitors by butyrate prevents cell cycle progression by failing to inactivate Rb .
	manualset3
131002	3	406123	13	NULL	NULL	0	NULL	downregulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of butyrate 's effect on D-type cyclins , downregulation of G1-specific cdks and upregulation of cdk inhibitors by butyrate prevents cell cycle progression by failing to inactivate Rb .
	manualset3
131003	4	406123	13	NULL	NULL	0	NULL	G1-specific cdks	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of butyrate 's effect on D-type cyclins , downregulation of G1-specific cdks and upregulation of cdk inhibitors by butyrate prevents cell cycle progression by failing to inactivate Rb .
	manualset3
131004	5	406123	13	NULL	NULL	0	NULL	upregulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of butyrate 's effect on D-type cyclins , downregulation of G1-specific cdks and upregulation of cdk inhibitors by butyrate prevents cell cycle progression by failing to inactivate Rb .
	manualset3
131005	6	406123	13	NULL	NULL	NULL	NULL	cdk inhibitors	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Regardless of butyrate 's effect on D-type cyclins , downregulation of G1-specific cdks and upregulation of cdk inhibitors by butyrate prevents cell cycle progression by failing to inactivate Rb .
	manualset3
131006	7	406123	13	NULL	NULL	0	NULL	butyrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of butyrate 's effect on D-type cyclins , downregulation of G1-specific cdks and upregulation of cdk inhibitors by butyrate prevents cell cycle progression by failing to inactivate Rb .
	manualset3
131007	8	406123	13	NULL	NULL	0	NULL	cell cycle progression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of butyrate 's effect on D-type cyclins , downregulation of G1-specific cdks and upregulation of cdk inhibitors by butyrate prevents cell cycle progression by failing to inactivate Rb .
	manualset3
131008	9	406123	13	NULL	NULL	0	NULL	Rb	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of butyrate 's effect on D-type cyclins , downregulation of G1-specific cdks and upregulation of cdk inhibitors by butyrate prevents cell cycle progression by failing to inactivate Rb .
	manualset3
131000	1	406124	13	NULL	NULL	NULL	NULL	modern control systems 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A modern control systems approach is shown to improve the bandwidth of force estimation by three to four times which is corroborated experimentally .
	manualset3
131009	2	406124	13	NULL	NULL	0	NULL	approach	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A modern control systems approach is shown to improve the bandwidth of force estimation by three to four times which is corroborated experimentally .
	manualset3
131010	3	406124	13	NULL	NULL	0	NULL	bandwidth 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A modern control systems approach is shown to improve the bandwidth of force estimation by three to four times which is corroborated experimentally .
	manualset3
131011	4	406124	13	NULL	NULL	0	NULL	force	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A modern control systems approach is shown to improve the bandwidth of force estimation by three to four times which is corroborated experimentally .
	manualset3
131012	5	406124	13	NULL	NULL	0	NULL	estimation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A modern control systems approach is shown to improve the bandwidth of force estimation by three to four times which is corroborated experimentally .
	manualset3
131013	6	406124	13	NULL	NULL	0	NULL	three to four times	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A modern control systems approach is shown to improve the bandwidth of force estimation by three to four times which is corroborated experimentally .
	manualset3
131014	1	406125	13	NULL	NULL	0	NULL	method	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of method used the combined analysis supported a division of Autolytinae into three major clades : one with epigamous Autolytus ; a second comprising Autolytus and Myrianida with posterior scissiparity and gemmiparity ; and a third containing Proceraea , Procerastea , and Virchowia with anterior scissiparity .
	manualset3
131015	2	406125	13	NULL	NULL	0	NULL	combined analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of method used the combined analysis supported a division of Autolytinae into three major clades : one with epigamous Autolytus ; a second comprising Autolytus and Myrianida with posterior scissiparity and gemmiparity ; and a third containing Proceraea , Procerastea , and Virchowia with anterior scissiparity .
	manualset3
131016	3	406125	13	NULL	NULL	0	NULL	division 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of method used the combined analysis supported a division of Autolytinae into three major clades : one with epigamous Autolytus ; a second comprising Autolytus and Myrianida with posterior scissiparity and gemmiparity ; and a third containing Proceraea , Procerastea , and Virchowia with anterior scissiparity .
	manualset3
131017	4	406125	13	NULL	NULL	0	NULL	Autolytinae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of method used the combined analysis supported a division of Autolytinae into three major clades : one with epigamous Autolytus ; a second comprising Autolytus and Myrianida with posterior scissiparity and gemmiparity ; and a third containing Proceraea , Procerastea , and Virchowia with anterior scissiparity .
	manualset3
131018	5	406125	13	NULL	NULL	0	NULL	three major clades	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of method used the combined analysis supported a division of Autolytinae into three major clades : one with epigamous Autolytus ; a second comprising Autolytus and Myrianida with posterior scissiparity and gemmiparity ; and a third containing Proceraea , Procerastea , and Virchowia with anterior scissiparity .
	manualset3
131019	6	406125	13	NULL	NULL	0	NULL	epigamous Autolytus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of method used the combined analysis supported a division of Autolytinae into three major clades : one with epigamous Autolytus ; a second comprising Autolytus and Myrianida with posterior scissiparity and gemmiparity ; and a third containing Proceraea , Procerastea , and Virchowia with anterior scissiparity .
	manualset3
131020	7	406125	13	NULL	NULL	0	NULL	Autolytus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of method used the combined analysis supported a division of Autolytinae into three major clades : one with epigamous Autolytus ; a second comprising Autolytus and Myrianida with posterior scissiparity and gemmiparity ; and a third containing Proceraea , Procerastea , and Virchowia with anterior scissiparity .
	manualset3
131021	8	406125	13	NULL	NULL	0	NULL	Myrianida	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of method used the combined analysis supported a division of Autolytinae into three major clades : one with epigamous Autolytus ; a second comprising Autolytus and Myrianida with posterior scissiparity and gemmiparity ; and a third containing Proceraea , Procerastea , and Virchowia with anterior scissiparity .
	manualset3
131022	9	406125	13	NULL	NULL	0	NULL	posterior scissiparity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of method used the combined analysis supported a division of Autolytinae into three major clades : one with epigamous Autolytus ; a second comprising Autolytus and Myrianida with posterior scissiparity and gemmiparity ; and a third containing Proceraea , Procerastea , and Virchowia with anterior scissiparity .
	manualset3
131023	10	406125	13	NULL	NULL	0	NULL	gemmiparity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of method used the combined analysis supported a division of Autolytinae into three major clades : one with epigamous Autolytus ; a second comprising Autolytus and Myrianida with posterior scissiparity and gemmiparity ; and a third containing Proceraea , Procerastea , and Virchowia with anterior scissiparity .
	manualset3
131024	11	406125	13	NULL	NULL	0	NULL	Proceraea	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of method used the combined analysis supported a division of Autolytinae into three major clades : one with epigamous Autolytus ; a second comprising Autolytus and Myrianida with posterior scissiparity and gemmiparity ; and a third containing Proceraea , Procerastea , and Virchowia with anterior scissiparity .
	manualset3
131025	12	406125	13	NULL	NULL	0	NULL	Procerastea	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of method used the combined analysis supported a division of Autolytinae into three major clades : one with epigamous Autolytus ; a second comprising Autolytus and Myrianida with posterior scissiparity and gemmiparity ; and a third containing Proceraea , Procerastea , and Virchowia with anterior scissiparity .
	manualset3
131026	13	406125	13	NULL	NULL	0	NULL	Virchowia 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of method used the combined analysis supported a division of Autolytinae into three major clades : one with epigamous Autolytus ; a second comprising Autolytus and Myrianida with posterior scissiparity and gemmiparity ; and a third containing Proceraea , Procerastea , and Virchowia with anterior scissiparity .
	manualset3
131027	14	406125	13	NULL	NULL	0	NULL	anterior scissiparity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of method used the combined analysis supported a division of Autolytinae into three major clades : one with epigamous Autolytus ; a second comprising Autolytus and Myrianida with posterior scissiparity and gemmiparity ; and a third containing Proceraea , Procerastea , and Virchowia with anterior scissiparity .
	manualset3
131028	1	406126	13	NULL	NULL	0	NULL	population	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of population , adults from pupae that experienced prolonged dormancy were larger than counterparts emerging within 1year .
	manualset3
131029	2	406126	13	NULL	NULL	0	NULL	adults	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of population , adults from pupae that experienced prolonged dormancy were larger than counterparts emerging within 1year .
	manualset3
131030	3	406126	13	NULL	NULL	0	NULL	pupae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of population , adults from pupae that experienced prolonged dormancy were larger than counterparts emerging within 1year .
	manualset3
131031	4	406126	13	NULL	NULL	0	NULL	dormancy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of population , adults from pupae that experienced prolonged dormancy were larger than counterparts emerging within 1year .
	manualset3
131032	5	406126	13	NULL	NULL	0	NULL	counterparts	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of population , adults from pupae that experienced prolonged dormancy were larger than counterparts emerging within 1year .
	manualset3
131033	6	406126	13	NULL	NULL	0	NULL	1year 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of population , adults from pupae that experienced prolonged dormancy were larger than counterparts emerging within 1year .
	manualset3
131034	1	406127	13	NULL	NULL	0	NULL	nature 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of the nature of the underlying defect , a treatment that could reduce the rate of muscle protein degradation may be of therapeutic value in these conditions .
	manualset3
131035	2	406127	13	NULL	NULL	0	NULL	defect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of the nature of the underlying defect , a treatment that could reduce the rate of muscle protein degradation may be of therapeutic value in these conditions .
	manualset3
131036	3	406127	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of the nature of the underlying defect , a treatment that could reduce the rate of muscle protein degradation may be of therapeutic value in these conditions .
	manualset3
131037	4	406127	13	NULL	NULL	0	NULL	rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of the nature of the underlying defect , a treatment that could reduce the rate of muscle protein degradation may be of therapeutic value in these conditions .
	manualset3
131038	5	406127	13	NULL	NULL	0	NULL	muscle protein degradation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of the nature of the underlying defect , a treatment that could reduce the rate of muscle protein degradation may be of therapeutic value in these conditions .
	manualset3
131039	6	406127	13	NULL	NULL	0	NULL	therapeutic value	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of the nature of the underlying defect , a treatment that could reduce the rate of muscle protein degradation may be of therapeutic value in these conditions .
	manualset3
131040	7	406127	13	NULL	NULL	0	NULL	conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of the nature of the underlying defect , a treatment that could reduce the rate of muscle protein degradation may be of therapeutic value in these conditions .
	manualset3
131041	1	406128	13	NULL	NULL	0	NULL	paced site 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of the paced site , there was a range of coupling intervals during which testing stimuli elicited short runs of premature beats .
	manualset3
131042	2	406128	13	NULL	NULL	0	NULL	intervals	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of the paced site , there was a range of coupling intervals during which testing stimuli elicited short runs of premature beats .
	manualset3
131043	3	406128	13	NULL	NULL	0	NULL	testing stimuli	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of the paced site , there was a range of coupling intervals during which testing stimuli elicited short runs of premature beats .
	manualset3
131044	4	406128	13	NULL	NULL	NULL	NULL	short runs 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Regardless of the paced site , there was a range of coupling intervals during which testing stimuli elicited short runs of premature beats .
	manualset3
131045	5	406128	13	NULL	NULL	0	NULL	premature beats 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regardless of the paced site , there was a range of coupling intervals during which testing stimuli elicited short runs of premature beats .
	manualset3
131046	1	406129	13	NULL	NULL	0	NULL	foveolae	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Regenerated foveolae and glands consisted of large SMC and MNC and a few fibrillovesicular cells .
	manualset3
131047	2	406129	13	NULL	NULL	0	NULL	glands 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Regenerated foveolae and glands consisted of large SMC and MNC and a few fibrillovesicular cells .
	manualset3
131048	3	406129	13	NULL	NULL	0	NULL	SMC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Regenerated foveolae and glands consisted of large SMC and MNC and a few fibrillovesicular cells .
	manualset3
131049	4	406129	13	NULL	NULL	0	NULL	MNC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Regenerated foveolae and glands consisted of large SMC and MNC and a few fibrillovesicular cells .
	manualset3
131050	5	406129	13	NULL	NULL	0	NULL	fibrillovesicular cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Regenerated foveolae and glands consisted of large SMC and MNC and a few fibrillovesicular cells .
	manualset3
131051	1	406130	13	NULL	NULL	0	NULL	Regeneration 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regeneration of axons and synaptic complex formation rostral to the site of hemisection in the spinal cord of the monkey .
	manualset3
131052	2	406130	13	NULL	NULL	0	NULL	axons	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Regeneration of axons and synaptic complex formation rostral to the site of hemisection in the spinal cord of the monkey .
	manualset3
131053	3	406130	13	NULL	NULL	0	NULL	synaptic complex formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regeneration of axons and synaptic complex formation rostral to the site of hemisection in the spinal cord of the monkey .
	manualset3
131054	4	406130	13	NULL	NULL	0	NULL	site of hemisection	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Regeneration of axons and synaptic complex formation rostral to the site of hemisection in the spinal cord of the monkey .
	manualset3
131055	5	406130	13	NULL	NULL	0	NULL	spinal cord	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Regeneration of axons and synaptic complex formation rostral to the site of hemisection in the spinal cord of the monkey .
	manualset3
131056	6	406130	13	NULL	NULL	0	NULL	monkey	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Regeneration of axons and synaptic complex formation rostral to the site of hemisection in the spinal cord of the monkey .
	manualset3
131778	1	406131	13	NULL	NULL	0	NULL	Regimen A	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Regimen A consisted of an oral dose of 150 mg Ca as AAACa after each meal and 450 mg at bedtime ; B consisted of 300 mg after each meal and C was placebo .
	manualset3
131779	2	406131	13	NULL	NULL	0	NULL	oral dose	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Regimen A consisted of an oral dose of 150 mg Ca as AAACa after each meal and 450 mg at bedtime ; B consisted of 300 mg after each meal and C was placebo .
	manualset3
131780	3	406131	13	NULL	NULL	0	NULL	150 mg Ca	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Regimen A consisted of an oral dose of 150 mg Ca as AAACa after each meal and 450 mg at bedtime ; B consisted of 300 mg after each meal and C was placebo .
	manualset3
131781	4	406131	13	NULL	NULL	0	NULL	AAACa	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Regimen A consisted of an oral dose of 150 mg Ca as AAACa after each meal and 450 mg at bedtime ; B consisted of 300 mg after each meal and C was placebo .
	manualset3
131782	5	406131	13	NULL	NULL	0	NULL	meal 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Regimen A consisted of an oral dose of 150 mg Ca as AAACa after each meal and 450 mg at bedtime ; B consisted of 300 mg after each meal and C was placebo .
	manualset3
131783	6	406131	13	NULL	NULL	0	NULL	450 mg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Regimen A consisted of an oral dose of 150 mg Ca as AAACa after each meal and 450 mg at bedtime ; B consisted of 300 mg after each meal and C was placebo .
	manualset3
131784	7	406131	13	NULL	NULL	0	NULL	bedtime 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Regimen A consisted of an oral dose of 150 mg Ca as AAACa after each meal and 450 mg at bedtime ; B consisted of 300 mg after each meal and C was placebo .
	manualset3
131785	8	406131	13	NULL	NULL	0	NULL	Regimen B	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Regimen A consisted of an oral dose of 150 mg Ca as AAACa after each meal and 450 mg at bedtime ; B consisted of 300 mg after each meal and C was placebo .
	manualset3
131786	9	406131	13	NULL	NULL	0	NULL	300 mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Regimen A consisted of an oral dose of 150 mg Ca as AAACa after each meal and 450 mg at bedtime ; B consisted of 300 mg after each meal and C was placebo .
	manualset3
131787	10	406131	13	NULL	NULL	0	NULL	meal 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Regimen A consisted of an oral dose of 150 mg Ca as AAACa after each meal and 450 mg at bedtime ; B consisted of 300 mg after each meal and C was placebo .
	manualset3
131788	11	406131	13	NULL	NULL	0	NULL	Regimen C	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Regimen A consisted of an oral dose of 150 mg Ca as AAACa after each meal and 450 mg at bedtime ; B consisted of 300 mg after each meal and C was placebo .
	manualset3
131789	12	406131	13	NULL	NULL	NULL	NULL	placebo	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Regimen A consisted of an oral dose of 150 mg Ca as AAACa after each meal and 450 mg at bedtime ; B consisted of 300 mg after each meal and C was placebo .
	manualset3
131790	1	406132	13	NULL	NULL	0	NULL	Regio silylmetalation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Regio - and chemoselective silylmetalation of functionalized terminal alkenes .
	manualset3
131791	2	406132	13	NULL	NULL	0	NULL	chemoselective silylmetalation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Regio - and chemoselective silylmetalation of functionalized terminal alkenes .
	manualset3
131792	3	406132	13	NULL	NULL	0	NULL	alkenes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Regio - and chemoselective silylmetalation of functionalized terminal alkenes .
	manualset3
131793	1	406133	13	NULL	NULL	0	NULL	alterations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Region-specific alterations in dopamine and serotonin metabolism in brains of rats exposed to low levels of lead .
	manualset3
131794	2	406133	13	NULL	NULL	0	NULL	dopamine metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Region-specific alterations in dopamine and serotonin metabolism in brains of rats exposed to low levels of lead .
	manualset3
131795	3	406133	13	NULL	NULL	0	NULL	serotonin metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Region-specific alterations in dopamine and serotonin metabolism in brains of rats exposed to low levels of lead .
	manualset3
131796	4	406133	13	NULL	NULL	0	NULL	brains	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Region-specific alterations in dopamine and serotonin metabolism in brains of rats exposed to low levels of lead .
	manualset3
131797	5	406133	13	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Region-specific alterations in dopamine and serotonin metabolism in brains of rats exposed to low levels of lead .
	manualset3
131798	6	406133	13	NULL	NULL	0	NULL	levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Region-specific alterations in dopamine and serotonin metabolism in brains of rats exposed to low levels of lead .
	manualset3
131799	7	406133	13	NULL	NULL	0	NULL	lead	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Region-specific alterations in dopamine and serotonin metabolism in brains of rats exposed to low levels of lead .
	manualset3
131800	1	406134	13	NULL	NULL	NULL	NULL	Regional glycerol changes	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Regional and temporal glycerol changes induced by forebrain ischemia in gerbils .
	manualset3
131801	2	406134	13	NULL	NULL	NULL	NULL	temporal glycerol changes 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Regional and temporal glycerol changes induced by forebrain ischemia in gerbils .
	manualset3
131802	3	406134	13	NULL	NULL	0	NULL	forebrain ischemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Regional and temporal glycerol changes induced by forebrain ischemia in gerbils .
	manualset3
131803	4	406134	13	NULL	NULL	0	NULL	gerbils	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Regional and temporal glycerol changes induced by forebrain ischemia in gerbils .
	manualset3
131804	1	406135	13	NULL	NULL	0	NULL	Regional blockade	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Regional blockade in patients with a history of a seizure disorder .
	manualset3
131805	2	406135	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Regional blockade in patients with a history of a seizure disorder .
	manualset3
131806	3	406135	13	NULL	NULL	0	NULL	history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Regional blockade in patients with a history of a seizure disorder .
	manualset3
131807	4	406135	13	NULL	NULL	0	NULL	seizure disorder	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Regional blockade in patients with a history of a seizure disorder .
	manualset3
131808	1	406136	13	NULL	NULL	0	NULL	Regional sensitivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regional sensitivity of cyclic AMP and cyclic GMP in rat brain to central cholinergic stimulation .
	manualset3
131809	2	406136	13	NULL	NULL	0	NULL	cyclic AMP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Regional sensitivity of cyclic AMP and cyclic GMP in rat brain to central cholinergic stimulation .
	manualset3
131810	3	406136	13	NULL	NULL	0	NULL	cyclic GMP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Regional sensitivity of cyclic AMP and cyclic GMP in rat brain to central cholinergic stimulation .
	manualset3
131811	4	406136	13	NULL	NULL	0	NULL	rat brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Regional sensitivity of cyclic AMP and cyclic GMP in rat brain to central cholinergic stimulation .
	manualset3
131812	5	406136	13	NULL	NULL	0	NULL	central cholinergic stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regional sensitivity of cyclic AMP and cyclic GMP in rat brain to central cholinergic stimulation .
	manualset3
131813	1	406137	13	NULL	NULL	0	NULL	alterations 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regionally selective alterations in local cerebral glucose utilization evoked by charybdotoxin , a blocker of central voltage-activated K + - channels .
	manualset3
131814	2	406137	13	NULL	NULL	0	NULL	local cerebral glucose utilization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regionally selective alterations in local cerebral glucose utilization evoked by charybdotoxin , a blocker of central voltage-activated K + - channels .
	manualset3
131815	3	406137	13	NULL	NULL	0	NULL	charybdotoxin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Regionally selective alterations in local cerebral glucose utilization evoked by charybdotoxin , a blocker of central voltage-activated K + - channels .
	manualset3
131816	4	406137	13	NULL	NULL	0	NULL	blocker	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Regionally selective alterations in local cerebral glucose utilization evoked by charybdotoxin , a blocker of central voltage-activated K + - channels .
	manualset3
134866	5	406137	13	NULL	NULL	0	NULL	central voltage-activated K + - channels	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Regionally selective alterations in local cerebral glucose utilization evoked by charybdotoxin , a blocker of central voltage-activated K + - channels .
	manualset3
131817	5	406138	13	NULL	NULL	NULL	NULL	Regions	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Regions in the Z5 mating gene of Schizophyllum commune involved in Y-Z binding and recognition .
	manualset3
131818	6	406138	13	NULL	NULL	0	NULL	Z5 mating gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Regions in the Z5 mating gene of Schizophyllum commune involved in Y-Z binding and recognition .
	manualset3
131819	7	406138	13	NULL	NULL	0	NULL	Schizophyllum commune	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Regions in the Z5 mating gene of Schizophyllum commune involved in Y-Z binding and recognition .
	manualset3
131820	8	406138	13	NULL	NULL	0	NULL	Y-Z binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regions in the Z5 mating gene of Schizophyllum commune involved in Y-Z binding and recognition .
	manualset3
131821	9	406138	13	NULL	NULL	0	NULL	recognition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regions in the Z5 mating gene of Schizophyllum commune involved in Y-Z binding and recognition .
	manualset3
131822	1	406139	13	NULL	NULL	0	NULL	Regression analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Regression analysis of the enzymatic assay ( y ) vs. the HPLC method ( x ) produced the following relation : y = 0.964 x +0.090 ( n = 262 , Sy , x = 6.37 ng/mL ) .
	manualset3
131823	2	406139	13	NULL	NULL	0	NULL	enzymatic assay ( y )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Regression analysis of the enzymatic assay ( y ) vs. the HPLC method ( x ) produced the following relation : y = 0.964 x +0.090 ( n = 262 , Sy , x = 6.37 ng/mL ) .
	manualset3
131824	3	406139	13	NULL	NULL	0	NULL	HPLC method ( x )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Regression analysis of the enzymatic assay ( y ) vs. the HPLC method ( x ) produced the following relation : y = 0.964 x +0.090 ( n = 262 , Sy , x = 6.37 ng/mL ) .
	manualset3
131825	4	406139	13	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Regression analysis of the enzymatic assay ( y ) vs. the HPLC method ( x ) produced the following relation : y = 0.964 x +0.090 ( n = 262 , Sy , x = 6.37 ng/mL ) .
	manualset3
131826	5	406139	13	NULL	NULL	0	NULL	y = 0.964 x +0.090	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Regression analysis of the enzymatic assay ( y ) vs. the HPLC method ( x ) produced the following relation : y = 0.964 x +0.090 ( n = 262 , Sy , x = 6.37 ng/mL ) .
	manualset3
131827	6	406139	13	NULL	NULL	0	NULL	n = 262 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Regression analysis of the enzymatic assay ( y ) vs. the HPLC method ( x ) produced the following relation : y = 0.964 x +0.090 ( n = 262 , Sy , x = 6.37 ng/mL ) .
	manualset3
131828	7	406139	13	NULL	NULL	0	NULL	Sy , x = 6.37 ng/mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Regression analysis of the enzymatic assay ( y ) vs. the HPLC method ( x ) produced the following relation : y = 0.964 x +0.090 ( n = 262 , Sy , x = 6.37 ng/mL ) .
	manualset3
131829	1	406140	13	NULL	NULL	0	NULL	Regression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Regression of metastatic lesions of breast carcinoma following sterilization .
	manualset3
131830	2	406140	13	NULL	NULL	0	NULL	metastatic lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Regression of metastatic lesions of breast carcinoma following sterilization .
	manualset3
131831	3	406140	13	NULL	NULL	0	NULL	breast carcinoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Regression of metastatic lesions of breast carcinoma following sterilization .
	manualset3
131832	4	406140	13	NULL	NULL	0	NULL	sterilization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Regression of metastatic lesions of breast carcinoma following sterilization .
	manualset3
131833	1	406141	13	NULL	NULL	0	NULL	Regression 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Regression of posterior uveal malignant melanomas after cobalt plaque radiotherapy .
	manualset3
131834	2	406141	13	NULL	NULL	0	NULL	posterior uveal malignant melanomas 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Regression of posterior uveal malignant melanomas after cobalt plaque radiotherapy .
	manualset3
131835	3	406141	13	NULL	NULL	0	NULL	cobalt plaque radiotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Regression of posterior uveal malignant melanomas after cobalt plaque radiotherapy .
	manualset3
131836	1	406142	13	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A modified model in which a correction factor is introduced was applied to the problem and proved to give a reliable calculation method for INR on Normotest .
	manualset3
131837	2	406142	13	NULL	NULL	0	NULL	correction factor	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A modified model in which a correction factor is introduced was applied to the problem and proved to give a reliable calculation method for INR on Normotest .
	manualset3
131838	3	406142	13	NULL	NULL	0	NULL	problem	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A modified model in which a correction factor is introduced was applied to the problem and proved to give a reliable calculation method for INR on Normotest .
	manualset3
131839	4	406142	13	NULL	NULL	NULL	NULL	calculation method	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A modified model in which a correction factor is introduced was applied to the problem and proved to give a reliable calculation method for INR on Normotest .
	manualset3
131840	5	406142	13	NULL	NULL	0	NULL	INR	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A modified model in which a correction factor is introduced was applied to the problem and proved to give a reliable calculation method for INR on Normotest .
	manualset3
131841	6	406142	13	NULL	NULL	NULL	NULL	Normotest	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A modified model in which a correction factor is introduced was applied to the problem and proved to give a reliable calculation method for INR on Normotest .
	manualset3
131842	1	406143	13	NULL	NULL	0	NULL	Regular administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular administration of IVIG overcomes the high risk of infections due to the severe immunodeficiency and the intensive immunosuppressive therapy .
	manualset3
131843	2	406143	13	NULL	NULL	0	NULL	IVIG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular administration of IVIG overcomes the high risk of infections due to the severe immunodeficiency and the intensive immunosuppressive therapy .
	manualset3
131844	3	406143	13	NULL	NULL	0	NULL	risk of infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular administration of IVIG overcomes the high risk of infections due to the severe immunodeficiency and the intensive immunosuppressive therapy .
	manualset3
131845	4	406143	13	NULL	NULL	0	NULL	severe immunodeficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular administration of IVIG overcomes the high risk of infections due to the severe immunodeficiency and the intensive immunosuppressive therapy .
	manualset3
131846	5	406143	13	NULL	NULL	0	NULL	intensive immunosuppressive therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular administration of IVIG overcomes the high risk of infections due to the severe immunodeficiency and the intensive immunosuppressive therapy .
	manualset3
131847	1	406144	13	NULL	NULL	0	NULL	Regular nucleosomal arrays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular nucleosomal arrays emanate more asymmetrically-mainly codirectionally with transcription-from promoter nucleosome-depleted regions , but promoters harboring the histone variant H2A .
	manualset3
131848	2	406144	13	NULL	NULL	0	NULL	transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular nucleosomal arrays emanate more asymmetrically-mainly codirectionally with transcription-from promoter nucleosome-depleted regions , but promoters harboring the histone variant H2A .
	manualset3
131849	3	406144	13	NULL	NULL	0	NULL	promoter nucleosome-depleted regions	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular nucleosomal arrays emanate more asymmetrically-mainly codirectionally with transcription-from promoter nucleosome-depleted regions , but promoters harboring the histone variant H2A .
	manualset3
131850	4	406144	13	NULL	NULL	0	NULL	promoters	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular nucleosomal arrays emanate more asymmetrically-mainly codirectionally with transcription-from promoter nucleosome-depleted regions , but promoters harboring the histone variant H2A .
	manualset3
131851	5	406144	13	NULL	NULL	0	NULL	histone variant H2A	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular nucleosomal arrays emanate more asymmetrically-mainly codirectionally with transcription-from promoter nucleosome-depleted regions , but promoters harboring the histone variant H2A .
	manualset3
131852	1	406145	13	NULL	NULL	0	NULL	Regular patterns	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular patterns of actomyosin interactions arise when ribbons are aligned with myosin thick filaments , because the repeat distance of the myosin lattice ( 429 A ) is an integral multiple of the subunit repeat in the ribbon ( 35.7 A ) .
	manualset3
131853	2	406145	13	NULL	NULL	0	NULL	actomyosin interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular patterns of actomyosin interactions arise when ribbons are aligned with myosin thick filaments , because the repeat distance of the myosin lattice ( 429 A ) is an integral multiple of the subunit repeat in the ribbon ( 35.7 A ) .
	manualset3
131854	3	406145	13	NULL	NULL	0	NULL	ribbons	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular patterns of actomyosin interactions arise when ribbons are aligned with myosin thick filaments , because the repeat distance of the myosin lattice ( 429 A ) is an integral multiple of the subunit repeat in the ribbon ( 35.7 A ) .
	manualset3
131855	4	406145	13	NULL	NULL	0	NULL	myosin thick filaments	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular patterns of actomyosin interactions arise when ribbons are aligned with myosin thick filaments , because the repeat distance of the myosin lattice ( 429 A ) is an integral multiple of the subunit repeat in the ribbon ( 35.7 A ) .
	manualset3
131856	5	406145	13	NULL	NULL	0	NULL	repeat distance	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular patterns of actomyosin interactions arise when ribbons are aligned with myosin thick filaments , because the repeat distance of the myosin lattice ( 429 A ) is an integral multiple of the subunit repeat in the ribbon ( 35.7 A ) .
	manualset3
131857	6	406145	13	NULL	NULL	NULL	NULL	myosin lattice 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Regular patterns of actomyosin interactions arise when ribbons are aligned with myosin thick filaments , because the repeat distance of the myosin lattice ( 429 A ) is an integral multiple of the subunit repeat in the ribbon ( 35.7 A ) .
	manualset3
131858	7	406145	13	NULL	NULL	0	NULL	subunit repeat 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular patterns of actomyosin interactions arise when ribbons are aligned with myosin thick filaments , because the repeat distance of the myosin lattice ( 429 A ) is an integral multiple of the subunit repeat in the ribbon ( 35.7 A ) .
	manualset3
131859	8	406145	13	NULL	NULL	NULL	NULL	ribbon	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Regular patterns of actomyosin interactions arise when ribbons are aligned with myosin thick filaments , because the repeat distance of the myosin lattice ( 429 A ) is an integral multiple of the subunit repeat in the ribbon ( 35.7 A ) .
	manualset3
131860	9	406145	13	NULL	NULL	0	NULL	429 A 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular patterns of actomyosin interactions arise when ribbons are aligned with myosin thick filaments , because the repeat distance of the myosin lattice ( 429 A ) is an integral multiple of the subunit repeat in the ribbon ( 35.7 A ) .
	manualset3
131861	10	406145	13	NULL	NULL	0	NULL	35.7 A	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular patterns of actomyosin interactions arise when ribbons are aligned with myosin thick filaments , because the repeat distance of the myosin lattice ( 429 A ) is an integral multiple of the subunit repeat in the ribbon ( 35.7 A ) .
	manualset3
131862	1	406146	13	NULL	NULL	NULL	NULL	Regular physical activity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Regular physical activity has been shown to protect against diverse components of the frailty syndrome in men and women of all ages and frailty is not a contra-indication to physical activity , rather it may be one of the most important reasons to prescribe physical exercise .
	manualset3
131863	2	406146	13	NULL	NULL	0	NULL	diverse components	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular physical activity has been shown to protect against diverse components of the frailty syndrome in men and women of all ages and frailty is not a contra-indication to physical activity , rather it may be one of the most important reasons to prescribe physical exercise .
	manualset3
131864	3	406146	13	NULL	NULL	0	NULL	frailty syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular physical activity has been shown to protect against diverse components of the frailty syndrome in men and women of all ages and frailty is not a contra-indication to physical activity , rather it may be one of the most important reasons to prescribe physical exercise .
	manualset3
131865	4	406146	13	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular physical activity has been shown to protect against diverse components of the frailty syndrome in men and women of all ages and frailty is not a contra-indication to physical activity , rather it may be one of the most important reasons to prescribe physical exercise .
	manualset3
131866	5	406146	13	NULL	NULL	0	NULL	women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular physical activity has been shown to protect against diverse components of the frailty syndrome in men and women of all ages and frailty is not a contra-indication to physical activity , rather it may be one of the most important reasons to prescribe physical exercise .
	manualset3
131867	6	406146	13	NULL	NULL	0	NULL	ages	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular physical activity has been shown to protect against diverse components of the frailty syndrome in men and women of all ages and frailty is not a contra-indication to physical activity , rather it may be one of the most important reasons to prescribe physical exercise .
	manualset3
131868	7	406146	13	NULL	NULL	0	NULL	frailty 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular physical activity has been shown to protect against diverse components of the frailty syndrome in men and women of all ages and frailty is not a contra-indication to physical activity , rather it may be one of the most important reasons to prescribe physical exercise .
	manualset3
131869	8	406146	13	NULL	NULL	0	NULL	contra-indication	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular physical activity has been shown to protect against diverse components of the frailty syndrome in men and women of all ages and frailty is not a contra-indication to physical activity , rather it may be one of the most important reasons to prescribe physical exercise .
	manualset3
131870	9	406146	13	NULL	NULL	0	NULL	physical activity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular physical activity has been shown to protect against diverse components of the frailty syndrome in men and women of all ages and frailty is not a contra-indication to physical activity , rather it may be one of the most important reasons to prescribe physical exercise .
	manualset3
131871	10	406146	13	NULL	NULL	0	NULL	reasons 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular physical activity has been shown to protect against diverse components of the frailty syndrome in men and women of all ages and frailty is not a contra-indication to physical activity , rather it may be one of the most important reasons to prescribe physical exercise .
	manualset3
131872	11	406146	13	NULL	NULL	0	NULL	physical exercise	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular physical activity has been shown to protect against diverse components of the frailty syndrome in men and women of all ages and frailty is not a contra-indication to physical activity , rather it may be one of the most important reasons to prescribe physical exercise .
	manualset3
131873	1	406147	13	NULL	NULL	0	NULL	Regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation and deregulation of human IgE synthesis .
	manualset3
131874	2	406147	13	NULL	NULL	0	NULL	deregulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation and deregulation of human IgE synthesis .
	manualset3
131875	3	406147	13	NULL	NULL	0	NULL	human IgE synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation and deregulation of human IgE synthesis .
	manualset3
131876	1	406148	13	NULL	NULL	0	NULL	Regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation in rDNA-deficient Drosophila melanogaster .
	manualset3
131877	2	406148	13	NULL	NULL	0	NULL	rDNA-deficient Drosophila melanogaster	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation in rDNA-deficient Drosophila melanogaster .
	manualset3
131878	1	406149	13	NULL	NULL	0	NULL	Regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of NAD and NADP synthesis in human red cell .
	manualset3
131879	2	406149	13	NULL	NULL	0	NULL	NAD synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of NAD and NADP synthesis in human red cell .
	manualset3
131880	3	406149	13	NULL	NULL	0	NULL	NADP synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of NAD and NADP synthesis in human red cell .
	manualset3
131881	4	406149	13	NULL	NULL	0	NULL	human red cell 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of NAD and NADP synthesis in human red cell .
	manualset3
131882	1	406150	13	NULL	NULL	0	NULL	Regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of Na ( + ) - K ( + ) - ATPase by cAMP-dependent protein kinase anchored on membrane via its anchoring protein .
	manualset3
131883	2	406150	13	NULL	NULL	0	NULL	Na ( + ) - K ( + ) - ATPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of Na ( + ) - K ( + ) - ATPase by cAMP-dependent protein kinase anchored on membrane via its anchoring protein .
	manualset3
131884	3	406150	13	NULL	NULL	0	NULL	cAMP-dependent protein kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of Na ( + ) - K ( + ) - ATPase by cAMP-dependent protein kinase anchored on membrane via its anchoring protein .
	manualset3
131885	4	406150	13	NULL	NULL	0	NULL	membrane 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of Na ( + ) - K ( + ) - ATPase by cAMP-dependent protein kinase anchored on membrane via its anchoring protein .
	manualset3
131886	5	406150	13	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of Na ( + ) - K ( + ) - ATPase by cAMP-dependent protein kinase anchored on membrane via its anchoring protein .
	manualset3
131887	1	406151	13	NULL	NULL	0	NULL	Regulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of UDP-galactose : ceramide galactosyltransferase and UDP-glucose : ceramide glucosyltransferase after crush and transection nerve injury .
	manualset3
131888	2	406151	13	NULL	NULL	0	NULL	UDP-galactose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of UDP-galactose : ceramide galactosyltransferase and UDP-glucose : ceramide glucosyltransferase after crush and transection nerve injury .
	manualset3
131889	3	406151	13	NULL	NULL	0	NULL	ceramide galactosyltransferase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of UDP-galactose : ceramide galactosyltransferase and UDP-glucose : ceramide glucosyltransferase after crush and transection nerve injury .
	manualset3
131890	4	406151	13	NULL	NULL	0	NULL	UDP-glucose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of UDP-galactose : ceramide galactosyltransferase and UDP-glucose : ceramide glucosyltransferase after crush and transection nerve injury .
	manualset3
131891	5	406151	13	NULL	NULL	0	NULL	ceramide glucosyltransferase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of UDP-galactose : ceramide galactosyltransferase and UDP-glucose : ceramide glucosyltransferase after crush and transection nerve injury .
	manualset3
131892	6	406151	13	NULL	NULL	0	NULL	crush 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of UDP-galactose : ceramide galactosyltransferase and UDP-glucose : ceramide glucosyltransferase after crush and transection nerve injury .
	manualset3
131893	7	406151	13	NULL	NULL	0	NULL	 transection nerve injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of UDP-galactose : ceramide galactosyltransferase and UDP-glucose : ceramide glucosyltransferase after crush and transection nerve injury .
	manualset3
131894	1	406152	13	NULL	NULL	0	NULL	Regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of alternative pathway complement activation by glycosaminoglycans : specificity of the polyanion binding site on factor H .
	manualset3
131895	2	406152	13	NULL	NULL	0	NULL	alternative pathway complement activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of alternative pathway complement activation by glycosaminoglycans : specificity of the polyanion binding site on factor H .
	manualset3
131896	3	406152	13	NULL	NULL	0	NULL	glycosaminoglycans	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of alternative pathway complement activation by glycosaminoglycans : specificity of the polyanion binding site on factor H .
	manualset3
131897	4	406152	13	NULL	NULL	0	NULL	specificity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of alternative pathway complement activation by glycosaminoglycans : specificity of the polyanion binding site on factor H .
	manualset3
131898	5	406152	13	NULL	NULL	0	NULL	polyanion binding site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of alternative pathway complement activation by glycosaminoglycans : specificity of the polyanion binding site on factor H .
	manualset3
131899	6	406152	13	NULL	NULL	0	NULL	factor H	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of alternative pathway complement activation by glycosaminoglycans : specificity of the polyanion binding site on factor H .
	manualset3
131900	1	406153	13	NULL	NULL	0	NULL	Regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of differentiation of the dimorphic fungus Paecilomyces viridis by nitrogen sources , antibiotics and metabolic inhibitors .
	manualset3
131901	2	406153	13	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of differentiation of the dimorphic fungus Paecilomyces viridis by nitrogen sources , antibiotics and metabolic inhibitors .
	manualset3
131902	3	406153	13	NULL	NULL	0	NULL	dimorphic fungus Paecilomyces viridis 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of differentiation of the dimorphic fungus Paecilomyces viridis by nitrogen sources , antibiotics and metabolic inhibitors .
	manualset3
131903	4	406153	13	NULL	NULL	0	NULL	nitrogen sources	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of differentiation of the dimorphic fungus Paecilomyces viridis by nitrogen sources , antibiotics and metabolic inhibitors .
	manualset3
131904	5	406153	13	NULL	NULL	0	NULL	antibiotics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of differentiation of the dimorphic fungus Paecilomyces viridis by nitrogen sources , antibiotics and metabolic inhibitors .
	manualset3
131905	6	406153	13	NULL	NULL	0	NULL	metabolic inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of differentiation of the dimorphic fungus Paecilomyces viridis by nitrogen sources , antibiotics and metabolic inhibitors .
	manualset3
131906	1	406154	13	NULL	NULL	0	NULL	Regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of induction by GLP1 , and localized cell surface receptor in Caenorhabditis elegans .
	manualset3
131907	2	406154	13	NULL	NULL	0	NULL	induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of induction by GLP1 , and localized cell surface receptor in Caenorhabditis elegans .
	manualset3
131908	3	406154	13	NULL	NULL	0	NULL	GLP1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of induction by GLP1 , and localized cell surface receptor in Caenorhabditis elegans .
	manualset3
131909	4	406154	13	NULL	NULL	0	NULL	cell surface receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of induction by GLP1 , and localized cell surface receptor in Caenorhabditis elegans .
	manualset3
131910	5	406154	13	NULL	NULL	0	NULL	Caenorhabditis elegans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of induction by GLP1 , and localized cell surface receptor in Caenorhabditis elegans .
	manualset3
131911	1	406155	13	NULL	NULL	0	NULL	Regulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of membrane transport through the endocytic pathway by rabGTPases .
	manualset3
131912	2	406155	13	NULL	NULL	0	NULL	membrane transport	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of membrane transport through the endocytic pathway by rabGTPases .
	manualset3
131913	3	406155	13	NULL	NULL	0	NULL	endocytic pathway 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of membrane transport through the endocytic pathway by rabGTPases .
	manualset3
131914	4	406155	13	NULL	NULL	0	NULL	rabGTPases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of membrane transport through the endocytic pathway by rabGTPases .
	manualset3
131918	1	406156	13	NULL	NULL	0	NULL	Regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of stromal sedoheptulose 1 , 7-bisphosphatase activity by pH and Mg2 + concentration .
	manualset3
131919	2	406156	13	NULL	NULL	0	NULL	stromal sedoheptulose 1 , 7-bisphosphatase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of stromal sedoheptulose 1 , 7-bisphosphatase activity by pH and Mg2 + concentration .
	manualset3
131920	3	406156	13	NULL	NULL	0	NULL	pH 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of stromal sedoheptulose 1 , 7-bisphosphatase activity by pH and Mg2 + concentration .
	manualset3
131921	4	406156	13	NULL	NULL	0	NULL	Mg2 + concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of stromal sedoheptulose 1 , 7-bisphosphatase activity by pH and Mg2 + concentration .
	manualset3
131922	1	406157	13	NULL	NULL	0	NULL	Regulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of substance P is similar to that of vasoactive intestinal peptide after axotomy or explantation of the rat superior cervical ganglion .
	manualset3
131923	2	406157	13	NULL	NULL	0	NULL	substance P	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of substance P is similar to that of vasoactive intestinal peptide after axotomy or explantation of the rat superior cervical ganglion .
	manualset3
131924	3	406157	13	NULL	NULL	0	NULL	vasoactive intestinal peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of substance P is similar to that of vasoactive intestinal peptide after axotomy or explantation of the rat superior cervical ganglion .
	manualset3
131925	4	406157	13	NULL	NULL	0	NULL	axotomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of substance P is similar to that of vasoactive intestinal peptide after axotomy or explantation of the rat superior cervical ganglion .
	manualset3
131926	5	406157	13	NULL	NULL	0	NULL	explantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of substance P is similar to that of vasoactive intestinal peptide after axotomy or explantation of the rat superior cervical ganglion .
	manualset3
131927	6	406157	13	NULL	NULL	0	NULL	rat superior cervical ganglion 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of substance P is similar to that of vasoactive intestinal peptide after axotomy or explantation of the rat superior cervical ganglion .
	manualset3
131928	1	406158	13	NULL	NULL	0	NULL	Regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of the human Fc epsilon RI alpha-chain distal promoter .
	manualset3
131929	2	406158	13	NULL	NULL	0	NULL	human Fc epsilon RI alpha-chain distal promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of the human Fc epsilon RI alpha-chain distal promoter .
	manualset3
131930	1	406159	13	NULL	NULL	0	NULL	Regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of the photorespiratory GLDPA gene in C ( 4 ) flaveria : an intricate interplay of transcriptional and posttranscriptional processes .
	manualset3
131931	2	406159	13	NULL	NULL	0	NULL	photorespiratory GLDPA gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of the photorespiratory GLDPA gene in C ( 4 ) flaveria : an intricate interplay of transcriptional and posttranscriptional processes .
	manualset3
131932	3	406159	13	NULL	NULL	0	NULL	C ( 4 ) flaveria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of the photorespiratory GLDPA gene in C ( 4 ) flaveria : an intricate interplay of transcriptional and posttranscriptional processes .
	manualset3
131933	4	406159	13	NULL	NULL	0	NULL	interplay	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of the photorespiratory GLDPA gene in C ( 4 ) flaveria : an intricate interplay of transcriptional and posttranscriptional processes .
	manualset3
131934	5	406159	13	NULL	NULL	0	NULL	transcriptional processes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of the photorespiratory GLDPA gene in C ( 4 ) flaveria : an intricate interplay of transcriptional and posttranscriptional processes .
	manualset3
131935	6	406159	13	NULL	NULL	0	NULL	posttranscriptional processes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of the photorespiratory GLDPA gene in C ( 4 ) flaveria : an intricate interplay of transcriptional and posttranscriptional processes .
	manualset3
131936	1	406160	13	NULL	NULL	0	NULL	Regulatory T cells ( Tregs )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulatory T cells ( Tregs ) play an essential role in the induction and maintenance of peripheral tolerance as well as prevention of autoimmunity by limiting the strength of the immune response of effector T cells .
	manualset3
131937	2	406160	13	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulatory T cells ( Tregs ) play an essential role in the induction and maintenance of peripheral tolerance as well as prevention of autoimmunity by limiting the strength of the immune response of effector T cells .
	manualset3
131938	3	406160	13	NULL	NULL	NULL	NULL	induction	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Regulatory T cells ( Tregs ) play an essential role in the induction and maintenance of peripheral tolerance as well as prevention of autoimmunity by limiting the strength of the immune response of effector T cells .
	manualset3
131939	4	406160	13	NULL	NULL	NULL	NULL	maintenance	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Regulatory T cells ( Tregs ) play an essential role in the induction and maintenance of peripheral tolerance as well as prevention of autoimmunity by limiting the strength of the immune response of effector T cells .
	manualset3
131940	5	406160	13	NULL	NULL	0	NULL	peripheral tolerance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulatory T cells ( Tregs ) play an essential role in the induction and maintenance of peripheral tolerance as well as prevention of autoimmunity by limiting the strength of the immune response of effector T cells .
	manualset3
131941	6	406160	13	NULL	NULL	0	NULL	prevention	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulatory T cells ( Tregs ) play an essential role in the induction and maintenance of peripheral tolerance as well as prevention of autoimmunity by limiting the strength of the immune response of effector T cells .
	manualset3
131942	7	406160	13	NULL	NULL	0	NULL	autoimmunity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulatory T cells ( Tregs ) play an essential role in the induction and maintenance of peripheral tolerance as well as prevention of autoimmunity by limiting the strength of the immune response of effector T cells .
	manualset3
131943	8	406160	13	NULL	NULL	0	NULL	strength 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulatory T cells ( Tregs ) play an essential role in the induction and maintenance of peripheral tolerance as well as prevention of autoimmunity by limiting the strength of the immune response of effector T cells .
	manualset3
131944	9	406160	13	NULL	NULL	0	NULL	immune response 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulatory T cells ( Tregs ) play an essential role in the induction and maintenance of peripheral tolerance as well as prevention of autoimmunity by limiting the strength of the immune response of effector T cells .
	manualset3
131945	10	406160	13	NULL	NULL	0	NULL	effector T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulatory T cells ( Tregs ) play an essential role in the induction and maintenance of peripheral tolerance as well as prevention of autoimmunity by limiting the strength of the immune response of effector T cells .
	manualset3
131946	1	406161	13	NULL	NULL	0	NULL	Regulatory kinetic behavior	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulatory kinetic behavior for both substrates is obtained with the modified enzyme at a lower pH , consistent with the downward shift in the pK of the ionizable groups , but sensitivity to cAMP activation is abolished by the modification .
	manualset3
131947	2	406161	13	NULL	NULL	0	NULL	substrates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulatory kinetic behavior for both substrates is obtained with the modified enzyme at a lower pH , consistent with the downward shift in the pK of the ionizable groups , but sensitivity to cAMP activation is abolished by the modification .
	manualset3
131948	3	406161	13	NULL	NULL	0	NULL	enzyme 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulatory kinetic behavior for both substrates is obtained with the modified enzyme at a lower pH , consistent with the downward shift in the pK of the ionizable groups , but sensitivity to cAMP activation is abolished by the modification .
	manualset3
131949	4	406161	13	NULL	NULL	0	NULL	pH	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulatory kinetic behavior for both substrates is obtained with the modified enzyme at a lower pH , consistent with the downward shift in the pK of the ionizable groups , but sensitivity to cAMP activation is abolished by the modification .
	manualset3
131950	5	406161	13	NULL	NULL	0	NULL	shift	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulatory kinetic behavior for both substrates is obtained with the modified enzyme at a lower pH , consistent with the downward shift in the pK of the ionizable groups , but sensitivity to cAMP activation is abolished by the modification .
	manualset3
131951	6	406161	13	NULL	NULL	0	NULL	pK	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulatory kinetic behavior for both substrates is obtained with the modified enzyme at a lower pH , consistent with the downward shift in the pK of the ionizable groups , but sensitivity to cAMP activation is abolished by the modification .
	manualset3
131952	7	406161	13	NULL	NULL	0	NULL	ionizable groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulatory kinetic behavior for both substrates is obtained with the modified enzyme at a lower pH , consistent with the downward shift in the pK of the ionizable groups , but sensitivity to cAMP activation is abolished by the modification .
	manualset3
131953	8	406161	13	NULL	NULL	0	NULL	sensitivity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulatory kinetic behavior for both substrates is obtained with the modified enzyme at a lower pH , consistent with the downward shift in the pK of the ionizable groups , but sensitivity to cAMP activation is abolished by the modification .
	manualset3
131954	9	406161	13	NULL	NULL	0	NULL	cAMP activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulatory kinetic behavior for both substrates is obtained with the modified enzyme at a lower pH , consistent with the downward shift in the pK of the ionizable groups , but sensitivity to cAMP activation is abolished by the modification .
	manualset3
131955	10	406161	13	NULL	NULL	0	NULL	modification 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulatory kinetic behavior for both substrates is obtained with the modified enzyme at a lower pH , consistent with the downward shift in the pK of the ionizable groups , but sensitivity to cAMP activation is abolished by the modification .
	manualset3
131956	1	406162	13	NULL	NULL	0	NULL	Rehabilitation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Rehabilitation of arm function after stroke .
	manualset3
131957	2	406162	13	NULL	NULL	0	NULL	arm function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rehabilitation of arm function after stroke .
	manualset3
131958	3	406162	13	NULL	NULL	0	NULL	stroke	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rehabilitation of arm function after stroke .
	manualset3
131959	1	406163	13	NULL	NULL	0	NULL	Rehabilitation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Rehabilitation of leprosy-affected persons extends beyond the physical domain of prevention and treatment of impairments .
	manualset3
131960	2	406163	13	NULL	NULL	0	NULL	leprosy-affected persons 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Rehabilitation of leprosy-affected persons extends beyond the physical domain of prevention and treatment of impairments .
	manualset3
131961	3	406163	13	NULL	NULL	0	NULL	physical domain	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Rehabilitation of leprosy-affected persons extends beyond the physical domain of prevention and treatment of impairments .
	manualset3
131962	4	406163	13	NULL	NULL	0	NULL	prevention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Rehabilitation of leprosy-affected persons extends beyond the physical domain of prevention and treatment of impairments .
	manualset3
131963	5	406163	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Rehabilitation of leprosy-affected persons extends beyond the physical domain of prevention and treatment of impairments .
	manualset3
131964	6	406163	13	NULL	NULL	0	NULL	impairments	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rehabilitation of leprosy-affected persons extends beyond the physical domain of prevention and treatment of impairments .
	manualset3
131965	1	406164	13	NULL	NULL	0	NULL	Rehabilitees	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Rehabilitees who have completed substance withdrawal treatment are among the special target groups for vocational rehabilitation measures .
	manualset3
131966	2	406164	13	NULL	NULL	0	NULL	substance withdrawal treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Rehabilitees who have completed substance withdrawal treatment are among the special target groups for vocational rehabilitation measures .
	manualset3
131967	3	406164	13	NULL	NULL	0	NULL	target groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Rehabilitees who have completed substance withdrawal treatment are among the special target groups for vocational rehabilitation measures .
	manualset3
131968	4	406164	13	NULL	NULL	0	NULL	vocational rehabilitation measures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Rehabilitees who have completed substance withdrawal treatment are among the special target groups for vocational rehabilitation measures .
	manualset3
131969	1	406165	13	NULL	NULL	0	NULL	effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reinforcing effect as a function of infusion speed in intravenous self-administration of nicotine in rhesus monkeys .
	manualset3
131970	2	406165	13	NULL	NULL	0	NULL	function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reinforcing effect as a function of infusion speed in intravenous self-administration of nicotine in rhesus monkeys .
	manualset3
131971	3	406165	13	NULL	NULL	0	NULL	infusion speed	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Reinforcing effect as a function of infusion speed in intravenous self-administration of nicotine in rhesus monkeys .
	manualset3
131972	4	406165	13	NULL	NULL	0	NULL	intravenous self-administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Reinforcing effect as a function of infusion speed in intravenous self-administration of nicotine in rhesus monkeys .
	manualset3
131973	5	406165	13	NULL	NULL	0	NULL	nicotine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Reinforcing effect as a function of infusion speed in intravenous self-administration of nicotine in rhesus monkeys .
	manualset3
131974	6	406165	13	NULL	NULL	0	NULL	rhesus monkeys	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Reinforcing effect as a function of infusion speed in intravenous self-administration of nicotine in rhesus monkeys .
	manualset3
131975	1	406166	13	NULL	NULL	0	NULL	monoclonal antibody 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A monoclonal antibody opsonic for M6 streptococci lost its ability to completely opsonize one of the size mutants in this study .
	manualset3
131976	2	406166	13	NULL	NULL	0	NULL	M6 streptococci	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A monoclonal antibody opsonic for M6 streptococci lost its ability to completely opsonize one of the size mutants in this study .
	manualset3
131977	3	406166	13	NULL	NULL	0	NULL	ability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A monoclonal antibody opsonic for M6 streptococci lost its ability to completely opsonize one of the size mutants in this study .
	manualset3
131978	4	406166	13	NULL	NULL	0	NULL	size mutants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A monoclonal antibody opsonic for M6 streptococci lost its ability to completely opsonize one of the size mutants in this study .
	manualset3
131979	5	406166	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A monoclonal antibody opsonic for M6 streptococci lost its ability to completely opsonize one of the size mutants in this study .
	manualset3
134868	6	406166	13	NULL	NULL	0	NULL	one 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A monoclonal antibody opsonic for M6 streptococci lost its ability to completely opsonize one of the size mutants in this study .
	manualset3
131980	1	406167	13	NULL	NULL	0	NULL	Relapse dynamics 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relapse dynamics during smoking cessation : Recurrent abstinence violation effects and lapse-relapse progression .
	manualset3
131981	2	406167	13	NULL	NULL	0	NULL	cessation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Relapse dynamics during smoking cessation : Recurrent abstinence violation effects and lapse-relapse progression .
	manualset3
131982	3	406167	13	NULL	NULL	0	NULL	Recurrent abstinence violation effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relapse dynamics during smoking cessation : Recurrent abstinence violation effects and lapse-relapse progression .
	manualset3
131983	4	406167	13	NULL	NULL	0	NULL	lapse-relapse progression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relapse dynamics during smoking cessation : Recurrent abstinence violation effects and lapse-relapse progression .
	manualset3
131984	1	406168	13	NULL	NULL	0	NULL	Relatedness 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Relatedness and Group Work scores were not correlated .
	manualset3
131985	2	406168	13	NULL	NULL	0	NULL	Group Work scores	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Relatedness and Group Work scores were not correlated .
	manualset3
131986	1	406169	13	NULL	NULL	0	NULL	Relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Relation between concentration of air pollution and cause-specific mortality : four-year exposures to nitrogen dioxide and particulate matter pollutants in 470 neighborhoods in Oslo , Norway .
	manualset3
131987	2	406169	13	NULL	NULL	0	NULL	concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Relation between concentration of air pollution and cause-specific mortality : four-year exposures to nitrogen dioxide and particulate matter pollutants in 470 neighborhoods in Oslo , Norway .
	manualset3
131988	3	406169	13	NULL	NULL	0	NULL	air pollution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Relation between concentration of air pollution and cause-specific mortality : four-year exposures to nitrogen dioxide and particulate matter pollutants in 470 neighborhoods in Oslo , Norway .
	manualset3
131989	4	406169	13	NULL	NULL	0	NULL	cause-specific mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relation between concentration of air pollution and cause-specific mortality : four-year exposures to nitrogen dioxide and particulate matter pollutants in 470 neighborhoods in Oslo , Norway .
	manualset3
131990	5	406169	13	NULL	NULL	0	NULL	four-year exposures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Relation between concentration of air pollution and cause-specific mortality : four-year exposures to nitrogen dioxide and particulate matter pollutants in 470 neighborhoods in Oslo , Norway .
	manualset3
131991	6	406169	13	NULL	NULL	0	NULL	nitrogen dioxide 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Relation between concentration of air pollution and cause-specific mortality : four-year exposures to nitrogen dioxide and particulate matter pollutants in 470 neighborhoods in Oslo , Norway .
	manualset3
131992	7	406169	13	NULL	NULL	0	NULL	particulate matter pollutants 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Relation between concentration of air pollution and cause-specific mortality : four-year exposures to nitrogen dioxide and particulate matter pollutants in 470 neighborhoods in Oslo , Norway .
	manualset3
131993	8	406169	13	NULL	NULL	0	NULL	470 neighborhoods	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Relation between concentration of air pollution and cause-specific mortality : four-year exposures to nitrogen dioxide and particulate matter pollutants in 470 neighborhoods in Oslo , Norway .
	manualset3
131994	9	406169	13	NULL	NULL	0	NULL	Oslo	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Relation between concentration of air pollution and cause-specific mortality : four-year exposures to nitrogen dioxide and particulate matter pollutants in 470 neighborhoods in Oslo , Norway .
	manualset3
131995	10	406169	13	NULL	NULL	0	NULL	Norway	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Relation between concentration of air pollution and cause-specific mortality : four-year exposures to nitrogen dioxide and particulate matter pollutants in 470 neighborhoods in Oslo , Norway .
	manualset3
131996	1	406170	13	NULL	NULL	0	NULL	Relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between Auxin and Membrane-Integrity in Tissue Senescence and Abscission .
	manualset3
131997	2	406170	13	NULL	NULL	0	NULL	Auxin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between Auxin and Membrane-Integrity in Tissue Senescence and Abscission .
	manualset3
131998	3	406170	13	NULL	NULL	0	NULL	Membrane-Integrity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between Auxin and Membrane-Integrity in Tissue Senescence and Abscission .
	manualset3
131999	4	406170	13	NULL	NULL	0	NULL	Tissue Senescence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between Auxin and Membrane-Integrity in Tissue Senescence and Abscission .
	manualset3
132000	5	406170	13	NULL	NULL	0	NULL	Abscission	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between Auxin and Membrane-Integrity in Tissue Senescence and Abscission .
	manualset3
132001	1	406171	13	NULL	NULL	0	NULL	Relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between CD40 ligand expression and B type natriuretic peptide levels in patients with chronic heart failure .
	manualset3
132002	2	406171	13	NULL	NULL	0	NULL	CD40 ligand expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between CD40 ligand expression and B type natriuretic peptide levels in patients with chronic heart failure .
	manualset3
132003	3	406171	13	NULL	NULL	0	NULL	B type natriuretic peptide levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between CD40 ligand expression and B type natriuretic peptide levels in patients with chronic heart failure .
	manualset3
132004	4	406171	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between CD40 ligand expression and B type natriuretic peptide levels in patients with chronic heart failure .
	manualset3
132005	5	406171	13	NULL	NULL	0	NULL	chronic heart failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between CD40 ligand expression and B type natriuretic peptide levels in patients with chronic heart failure .
	manualset3
132006	1	406172	13	NULL	NULL	0	NULL	Relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between HPLC fingerprints and invivo pharmacological effects of a traditional Chinese medicine : Radix Angelicae Dahuricae .
	manualset3
132007	2	406172	13	NULL	NULL	0	NULL	HPLC fingerprints	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between HPLC fingerprints and invivo pharmacological effects of a traditional Chinese medicine : Radix Angelicae Dahuricae .
	manualset3
132008	3	406172	13	NULL	NULL	0	NULL	pharmacological effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between HPLC fingerprints and invivo pharmacological effects of a traditional Chinese medicine : Radix Angelicae Dahuricae .
	manualset3
132009	4	406172	13	NULL	NULL	0	NULL	traditional Chinese medicine	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between HPLC fingerprints and invivo pharmacological effects of a traditional Chinese medicine : Radix Angelicae Dahuricae .
	manualset3
132010	5	406172	13	NULL	NULL	0	NULL	Radix Angelicae Dahuricae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between HPLC fingerprints and invivo pharmacological effects of a traditional Chinese medicine : Radix Angelicae Dahuricae .
	manualset3
132011	1	406173	13	NULL	NULL	0	NULL	Relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between muscle strength and vitamin D metabolites : are there therapeutic possibilities in the elderly ?
	manualset3
132012	2	406173	13	NULL	NULL	0	NULL	muscle strength	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between muscle strength and vitamin D metabolites : are there therapeutic possibilities in the elderly ?
	manualset3
132013	3	406173	13	NULL	NULL	0	NULL	vitamin D metabolites 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between muscle strength and vitamin D metabolites : are there therapeutic possibilities in the elderly ?
	manualset3
132014	4	406173	13	NULL	NULL	0	NULL	therapeutic possibilities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between muscle strength and vitamin D metabolites : are there therapeutic possibilities in the elderly ?
	manualset3
132015	5	406173	13	NULL	NULL	0	NULL	elderly	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between muscle strength and vitamin D metabolites : are there therapeutic possibilities in the elderly ?
	manualset3
132016	1	406174	13	NULL	NULL	0	NULL	Relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between oral health and mortality rate .
	manualset3
132017	2	406174	13	NULL	NULL	0	NULL	oral health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between oral health and mortality rate .
	manualset3
132018	3	406174	13	NULL	NULL	0	NULL	mortality rate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between oral health and mortality rate .
	manualset3
132019	1	406175	13	NULL	NULL	0	NULL	month	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A month ago we perfomed phacoecmulsofication cataract syrgery , because a cataract developed due to high doses of steroid therapy .
	manualset3
132020	2	406175	13	NULL	NULL	0	NULL	phacoecmulsofication cataract syrgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A month ago we perfomed phacoecmulsofication cataract syrgery , because a cataract developed due to high doses of steroid therapy .
	manualset3
132021	3	406175	13	NULL	NULL	0	NULL	cataract 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A month ago we perfomed phacoecmulsofication cataract syrgery , because a cataract developed due to high doses of steroid therapy .
	manualset3
132022	4	406175	13	NULL	NULL	0	NULL	doses	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A month ago we perfomed phacoecmulsofication cataract syrgery , because a cataract developed due to high doses of steroid therapy .
	manualset3
132023	5	406175	13	NULL	NULL	0	NULL	steroid therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A month ago we perfomed phacoecmulsofication cataract syrgery , because a cataract developed due to high doses of steroid therapy .
	manualset3
132024	1	406176	13	NULL	NULL	0	NULL	Relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between prematurity and the incidence of cerebral palsy ) .
	manualset3
132025	2	406176	13	NULL	NULL	0	NULL	prematurity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between prematurity and the incidence of cerebral palsy ) .
	manualset3
132026	3	406176	13	NULL	NULL	0	NULL	incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between prematurity and the incidence of cerebral palsy ) .
	manualset3
132027	4	406176	13	NULL	NULL	0	NULL	cerebral palsy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between prematurity and the incidence of cerebral palsy ) .
	manualset3
132028	1	406177	13	NULL	NULL	0	NULL	Relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between separation time of plasma from heparinized whole blood on plasma biochemical analytes of loggerhead sea turtles ( Caretta caretta ) .
	manualset3
132029	2	406177	13	NULL	NULL	0	NULL	separation time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between separation time of plasma from heparinized whole blood on plasma biochemical analytes of loggerhead sea turtles ( Caretta caretta ) .
	manualset3
132030	3	406177	13	NULL	NULL	0	NULL	plasma 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between separation time of plasma from heparinized whole blood on plasma biochemical analytes of loggerhead sea turtles ( Caretta caretta ) .
	manualset3
132031	4	406177	13	NULL	NULL	0	NULL	blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between separation time of plasma from heparinized whole blood on plasma biochemical analytes of loggerhead sea turtles ( Caretta caretta ) .
	manualset3
132032	5	406177	13	NULL	NULL	0	NULL	plasma biochemical analytes 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between separation time of plasma from heparinized whole blood on plasma biochemical analytes of loggerhead sea turtles ( Caretta caretta ) .
	manualset3
132033	6	406177	13	NULL	NULL	0	NULL	loggerhead sea turtles ( Caretta caretta ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between separation time of plasma from heparinized whole blood on plasma biochemical analytes of loggerhead sea turtles ( Caretta caretta ) .
	manualset3
132034	1	406178	13	NULL	NULL	0	NULL	Relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between the gingival sulcus depth and interleukin-1 isoform concentrations within the adjacent gingival tissue .
	manualset3
132035	2	406178	13	NULL	NULL	0	NULL	gingival sulcus depth	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between the gingival sulcus depth and interleukin-1 isoform concentrations within the adjacent gingival tissue .
	manualset3
132036	3	406178	13	NULL	NULL	0	NULL	interleukin-1 isoform concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between the gingival sulcus depth and interleukin-1 isoform concentrations within the adjacent gingival tissue .
	manualset3
132037	4	406178	13	NULL	NULL	0	NULL	gingival tissue 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between the gingival sulcus depth and interleukin-1 isoform concentrations within the adjacent gingival tissue .
	manualset3
132038	1	406179	13	NULL	NULL	0	NULL	Relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between the in vitro response of dendritic cells to Lactobacillus and prevention of tumorigenesis in the mouse .
	manualset3
132039	2	406179	13	NULL	NULL	0	NULL	 response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between the in vitro response of dendritic cells to Lactobacillus and prevention of tumorigenesis in the mouse .
	manualset3
132040	3	406179	13	NULL	NULL	0	NULL	dendritic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between the in vitro response of dendritic cells to Lactobacillus and prevention of tumorigenesis in the mouse .
	manualset3
132041	4	406179	13	NULL	NULL	0	NULL	Lactobacillus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between the in vitro response of dendritic cells to Lactobacillus and prevention of tumorigenesis in the mouse .
	manualset3
132042	5	406179	13	NULL	NULL	0	NULL	prevention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between the in vitro response of dendritic cells to Lactobacillus and prevention of tumorigenesis in the mouse .
	manualset3
132043	6	406179	13	NULL	NULL	0	NULL	tumorigenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between the in vitro response of dendritic cells to Lactobacillus and prevention of tumorigenesis in the mouse .
	manualset3
132044	7	406179	13	NULL	NULL	0	NULL	mouse	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between the in vitro response of dendritic cells to Lactobacillus and prevention of tumorigenesis in the mouse .
	manualset3
132045	1	406180	13	NULL	NULL	0	NULL	Relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship of balance and mobility to fall incidence in people with chronic stroke .
	manualset3
132046	2	406180	13	NULL	NULL	0	NULL	balance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship of balance and mobility to fall incidence in people with chronic stroke .
	manualset3
132047	3	406180	13	NULL	NULL	0	NULL	mobility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship of balance and mobility to fall incidence in people with chronic stroke .
	manualset3
132048	4	406180	13	NULL	NULL	0	NULL	incidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship of balance and mobility to fall incidence in people with chronic stroke .
	manualset3
132049	5	406180	13	NULL	NULL	0	NULL	people 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship of balance and mobility to fall incidence in people with chronic stroke .
	manualset3
132050	6	406180	13	NULL	NULL	0	NULL	chronic stroke	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship of balance and mobility to fall incidence in people with chronic stroke .
	manualset3
132051	1	406181	13	NULL	NULL	0	NULL	Relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship of exposure to organ donation information to attitudes , beliefs , and donation decisions of next of kin .
	manualset3
132052	2	406181	13	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship of exposure to organ donation information to attitudes , beliefs , and donation decisions of next of kin .
	manualset3
132053	3	406181	13	NULL	NULL	0	NULL	organ donation information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship of exposure to organ donation information to attitudes , beliefs , and donation decisions of next of kin .
	manualset3
132054	4	406181	13	NULL	NULL	0	NULL	attitudes	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship of exposure to organ donation information to attitudes , beliefs , and donation decisions of next of kin .
	manualset3
132055	5	406181	13	NULL	NULL	0	NULL	beliefs	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship of exposure to organ donation information to attitudes , beliefs , and donation decisions of next of kin .
	manualset3
132056	6	406181	13	NULL	NULL	0	NULL	donation decisions 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship of exposure to organ donation information to attitudes , beliefs , and donation decisions of next of kin .
	manualset3
132057	7	406181	13	NULL	NULL	0	NULL	kin	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship of exposure to organ donation information to attitudes , beliefs , and donation decisions of next of kin .
	manualset3
132058	1	406182	13	NULL	NULL	0	NULL	Relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship of radiologic and histologic signs of inflammation in human root-filled teeth .
	manualset3
132059	2	406182	13	NULL	NULL	0	NULL	radiologic signs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship of radiologic and histologic signs of inflammation in human root-filled teeth .
	manualset3
132060	3	406182	13	NULL	NULL	0	NULL	histologic signs 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship of radiologic and histologic signs of inflammation in human root-filled teeth .
	manualset3
132061	4	406182	13	NULL	NULL	0	NULL	inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship of radiologic and histologic signs of inflammation in human root-filled teeth .
	manualset3
132062	5	406182	13	NULL	NULL	0	NULL	human root-filled teeth	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship of radiologic and histologic signs of inflammation in human root-filled teeth .
	manualset3
132063	1	406183	13	NULL	NULL	0	NULL	Relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship of serum total calcium and albumin and total protein in owl monkeys ( Aotus nancymai ) .
	manualset3
132064	2	406183	13	NULL	NULL	NULL	NULL	serum total calcium 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Relationship of serum total calcium and albumin and total protein in owl monkeys ( Aotus nancymai ) .
	manualset3
132065	3	406183	13	NULL	NULL	0	NULL	albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship of serum total calcium and albumin and total protein in owl monkeys ( Aotus nancymai ) .
	manualset3
132066	4	406183	13	NULL	NULL	0	NULL	total protein 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship of serum total calcium and albumin and total protein in owl monkeys ( Aotus nancymai ) .
	manualset3
132067	5	406183	13	NULL	NULL	0	NULL	owl monkeys ( Aotus nancymai )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship of serum total calcium and albumin and total protein in owl monkeys ( Aotus nancymai ) .
	manualset3
132068	1	406184	13	NULL	NULL	0	NULL	Relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship of type 1 cannabinoid receptor availability in the human brain to novelty-seeking temperament .
	manualset3
132069	2	406184	13	NULL	NULL	0	NULL	type 1 cannabinoid receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship of type 1 cannabinoid receptor availability in the human brain to novelty-seeking temperament .
	manualset3
132070	3	406184	13	NULL	NULL	0	NULL	availability 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship of type 1 cannabinoid receptor availability in the human brain to novelty-seeking temperament .
	manualset3
132071	4	406184	13	NULL	NULL	0	NULL	human brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship of type 1 cannabinoid receptor availability in the human brain to novelty-seeking temperament .
	manualset3
132072	5	406184	13	NULL	NULL	0	NULL	temperament 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship of type 1 cannabinoid receptor availability in the human brain to novelty-seeking temperament .
	manualset3
132073	1	406185	13	NULL	NULL	0	NULL	mix	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A more creative mix of methodologies is needed , that goes hand in hand with a close collaboration between researchers from the social sciences and health sciences field .
	manualset3
132074	2	406185	13	NULL	NULL	0	NULL	methodologies	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A more creative mix of methodologies is needed , that goes hand in hand with a close collaboration between researchers from the social sciences and health sciences field .
	manualset3
132075	3	406185	13	NULL	NULL	0	NULL	collaboration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A more creative mix of methodologies is needed , that goes hand in hand with a close collaboration between researchers from the social sciences and health sciences field .
	manualset3
132076	4	406185	13	NULL	NULL	0	NULL	researchers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A more creative mix of methodologies is needed , that goes hand in hand with a close collaboration between researchers from the social sciences and health sciences field .
	manualset3
132077	5	406185	13	NULL	NULL	0	NULL	social sciences field	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A more creative mix of methodologies is needed , that goes hand in hand with a close collaboration between researchers from the social sciences and health sciences field .
	manualset3
132078	6	406185	13	NULL	NULL	0	NULL	health sciences field 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A more creative mix of methodologies is needed , that goes hand in hand with a close collaboration between researchers from the social sciences and health sciences field .
	manualset3
132079	1	406186	13	NULL	NULL	0	NULL	Relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationships between endorsement of rape myths , other attitudes , sexual behavior , and demographic variables were examined .
	manualset3
132080	2	406186	13	NULL	NULL	0	NULL	endorsement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationships between endorsement of rape myths , other attitudes , sexual behavior , and demographic variables were examined .
	manualset3
132081	3	406186	13	NULL	NULL	0	NULL	rape myths	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationships between endorsement of rape myths , other attitudes , sexual behavior , and demographic variables were examined .
	manualset3
132082	4	406186	13	NULL	NULL	0	NULL	attitudes	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationships between endorsement of rape myths , other attitudes , sexual behavior , and demographic variables were examined .
	manualset3
132083	5	406186	13	NULL	NULL	0	NULL	sexual behavior	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationships between endorsement of rape myths , other attitudes , sexual behavior , and demographic variables were examined .
	manualset3
132084	6	406186	13	NULL	NULL	0	NULL	demographic variables	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationships between endorsement of rape myths , other attitudes , sexual behavior , and demographic variables were examined .
	manualset3
132085	1	406187	13	NULL	NULL	0	NULL	 biological effectiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative biological effectiveness of 241Am relative to 192Ir for continuous low-dose-rate irradiation of BA1112 rat sarcomas .
	manualset3
132086	2	406187	13	NULL	NULL	0	NULL	241Am	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative biological effectiveness of 241Am relative to 192Ir for continuous low-dose-rate irradiation of BA1112 rat sarcomas .
	manualset3
132087	3	406187	13	NULL	NULL	0	NULL	192Ir 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative biological effectiveness of 241Am relative to 192Ir for continuous low-dose-rate irradiation of BA1112 rat sarcomas .
	manualset3
132088	4	406187	13	NULL	NULL	0	NULL	low-dose-rate irradiation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative biological effectiveness of 241Am relative to 192Ir for continuous low-dose-rate irradiation of BA1112 rat sarcomas .
	manualset3
132089	5	406187	13	NULL	NULL	0	NULL	BA1112 rat sarcomas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative biological effectiveness of 241Am relative to 192Ir for continuous low-dose-rate irradiation of BA1112 rat sarcomas .
	manualset3
132090	1	406188	13	NULL	NULL	0	NULL	cholesterol synthesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative cholesterol synthesis and absorption reflected respective absolute values during each diet in the apo E4 group ( r range +0.713 to +0.893 ; P & lt ; 0.05 for each ) , but only during HD ( r +0.594 ; P = 0.015 ) in the apo E2 + E3 group .
	manualset3
132091	2	406188	13	NULL	NULL	0	NULL	absorption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative cholesterol synthesis and absorption reflected respective absolute values during each diet in the apo E4 group ( r range +0.713 to +0.893 ; P & lt ; 0.05 for each ) , but only during HD ( r +0.594 ; P = 0.015 ) in the apo E2 + E3 group .
	manualset3
132092	3	406188	13	NULL	NULL	0	NULL	values 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative cholesterol synthesis and absorption reflected respective absolute values during each diet in the apo E4 group ( r range +0.713 to +0.893 ; P & lt ; 0.05 for each ) , but only during HD ( r +0.594 ; P = 0.015 ) in the apo E2 + E3 group .
	manualset3
132093	4	406188	13	NULL	NULL	0	NULL	diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative cholesterol synthesis and absorption reflected respective absolute values during each diet in the apo E4 group ( r range +0.713 to +0.893 ; P & lt ; 0.05 for each ) , but only during HD ( r +0.594 ; P = 0.015 ) in the apo E2 + E3 group .
	manualset3
132094	5	406188	13	NULL	NULL	0	NULL	apo E4 group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative cholesterol synthesis and absorption reflected respective absolute values during each diet in the apo E4 group ( r range +0.713 to +0.893 ; P & lt ; 0.05 for each ) , but only during HD ( r +0.594 ; P = 0.015 ) in the apo E2 + E3 group .
	manualset3
132095	6	406188	13	NULL	NULL	0	NULL	r range +0.713 to +0.893 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative cholesterol synthesis and absorption reflected respective absolute values during each diet in the apo E4 group ( r range +0.713 to +0.893 ; P & lt ; 0.05 for each ) , but only during HD ( r +0.594 ; P = 0.015 ) in the apo E2 + E3 group .
	manualset3
132096	7	406188	13	NULL	NULL	0	NULL	P & lt ; 0.05 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative cholesterol synthesis and absorption reflected respective absolute values during each diet in the apo E4 group ( r range +0.713 to +0.893 ; P & lt ; 0.05 for each ) , but only during HD ( r +0.594 ; P = 0.015 ) in the apo E2 + E3 group .
	manualset3
132097	8	406188	13	NULL	NULL	0	NULL	HD	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative cholesterol synthesis and absorption reflected respective absolute values during each diet in the apo E4 group ( r range +0.713 to +0.893 ; P & lt ; 0.05 for each ) , but only during HD ( r +0.594 ; P = 0.015 ) in the apo E2 + E3 group .
	manualset3
132098	9	406188	13	NULL	NULL	0	NULL	r +0.594	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative cholesterol synthesis and absorption reflected respective absolute values during each diet in the apo E4 group ( r range +0.713 to +0.893 ; P & lt ; 0.05 for each ) , but only during HD ( r +0.594 ; P = 0.015 ) in the apo E2 + E3 group .
	manualset3
132099	10	406188	13	NULL	NULL	0	NULL	P = 0.015 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative cholesterol synthesis and absorption reflected respective absolute values during each diet in the apo E4 group ( r range +0.713 to +0.893 ; P & lt ; 0.05 for each ) , but only during HD ( r +0.594 ; P = 0.015 ) in the apo E2 + E3 group .
	manualset3
132100	11	406188	13	NULL	NULL	0	NULL	apo E2 + E3 group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative cholesterol synthesis and absorption reflected respective absolute values during each diet in the apo E4 group ( r range +0.713 to +0.893 ; P & lt ; 0.05 for each ) , but only during HD ( r +0.594 ; P = 0.015 ) in the apo E2 + E3 group .
	manualset3
132101	1	406189	13	NULL	NULL	0	NULL	contraindications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative contraindications for treatment include osteolytic lesions , pending spinal cord compression or pathologic fracture , preexisting severe myelosuppression , urinary incontinence , inability to follow radiation safety precautions , and severe renal insufficiency .
	manualset3
132102	2	406189	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative contraindications for treatment include osteolytic lesions , pending spinal cord compression or pathologic fracture , preexisting severe myelosuppression , urinary incontinence , inability to follow radiation safety precautions , and severe renal insufficiency .
	manualset3
132103	3	406189	13	NULL	NULL	0	NULL	osteolytic lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative contraindications for treatment include osteolytic lesions , pending spinal cord compression or pathologic fracture , preexisting severe myelosuppression , urinary incontinence , inability to follow radiation safety precautions , and severe renal insufficiency .
	manualset3
132104	4	406189	13	NULL	NULL	0	NULL	spinal cord compression 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative contraindications for treatment include osteolytic lesions , pending spinal cord compression or pathologic fracture , preexisting severe myelosuppression , urinary incontinence , inability to follow radiation safety precautions , and severe renal insufficiency .
	manualset3
132105	5	406189	13	NULL	NULL	0	NULL	pathologic fracture	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative contraindications for treatment include osteolytic lesions , pending spinal cord compression or pathologic fracture , preexisting severe myelosuppression , urinary incontinence , inability to follow radiation safety precautions , and severe renal insufficiency .
	manualset3
132106	6	406189	13	NULL	NULL	0	NULL	severe myelosuppression 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative contraindications for treatment include osteolytic lesions , pending spinal cord compression or pathologic fracture , preexisting severe myelosuppression , urinary incontinence , inability to follow radiation safety precautions , and severe renal insufficiency .
	manualset3
132107	7	406189	13	NULL	NULL	0	NULL	urinary incontinence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative contraindications for treatment include osteolytic lesions , pending spinal cord compression or pathologic fracture , preexisting severe myelosuppression , urinary incontinence , inability to follow radiation safety precautions , and severe renal insufficiency .
	manualset3
132108	8	406189	13	NULL	NULL	0	NULL	inability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative contraindications for treatment include osteolytic lesions , pending spinal cord compression or pathologic fracture , preexisting severe myelosuppression , urinary incontinence , inability to follow radiation safety precautions , and severe renal insufficiency .
	manualset3
132109	9	406189	13	NULL	NULL	0	NULL	radiation safety precautions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative contraindications for treatment include osteolytic lesions , pending spinal cord compression or pathologic fracture , preexisting severe myelosuppression , urinary incontinence , inability to follow radiation safety precautions , and severe renal insufficiency .
	manualset3
132110	10	406189	13	NULL	NULL	0	NULL	severe renal insufficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative contraindications for treatment include osteolytic lesions , pending spinal cord compression or pathologic fracture , preexisting severe myelosuppression , urinary incontinence , inability to follow radiation safety precautions , and severe renal insufficiency .
	manualset3
132111	1	406190	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative expression of AgB1 was the highest in cysts , where calcification has initiated .
	manualset3
132112	2	406190	13	NULL	NULL	0	NULL	AgB1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative expression of AgB1 was the highest in cysts , where calcification has initiated .
	manualset3
132113	3	406190	13	NULL	NULL	0	NULL	cysts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative expression of AgB1 was the highest in cysts , where calcification has initiated .
	manualset3
132114	4	406190	13	NULL	NULL	0	NULL	calcification 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative expression of AgB1 was the highest in cysts , where calcification has initiated .
	manualset3
132115	1	406191	13	NULL	NULL	0	NULL	Relative frequency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative frequency of IVS10nt546 mutation in a Portuguese phenylketonuric population .
	manualset3
132116	2	406191	13	NULL	NULL	0	NULL	IVS10nt546 mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative frequency of IVS10nt546 mutation in a Portuguese phenylketonuric population .
	manualset3
132117	3	406191	13	NULL	NULL	0	NULL	Portuguese phenylketonuric population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative frequency of IVS10nt546 mutation in a Portuguese phenylketonuric population .
	manualset3
132118	1	406192	13	NULL	NULL	0	NULL	Relative levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative levels of - caryophyllene in whole plants in the panicle-formation stage and panicles in the flowering stage were much higher than that in stems and leaves in the flowering stage .
	manualset3
132119	2	406192	13	NULL	NULL	0	NULL	caryophyllene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative levels of - caryophyllene in whole plants in the panicle-formation stage and panicles in the flowering stage were much higher than that in stems and leaves in the flowering stage .
	manualset3
132120	3	406192	13	NULL	NULL	0	NULL	plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative levels of - caryophyllene in whole plants in the panicle-formation stage and panicles in the flowering stage were much higher than that in stems and leaves in the flowering stage .
	manualset3
132121	4	406192	13	NULL	NULL	0	NULL	panicle-formation stage	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative levels of - caryophyllene in whole plants in the panicle-formation stage and panicles in the flowering stage were much higher than that in stems and leaves in the flowering stage .
	manualset3
132122	5	406192	13	NULL	NULL	0	NULL	panicles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative levels of - caryophyllene in whole plants in the panicle-formation stage and panicles in the flowering stage were much higher than that in stems and leaves in the flowering stage .
	manualset3
132123	6	406192	13	NULL	NULL	0	NULL	flowering stage	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative levels of - caryophyllene in whole plants in the panicle-formation stage and panicles in the flowering stage were much higher than that in stems and leaves in the flowering stage .
	manualset3
132124	7	406192	13	NULL	NULL	0	NULL	stems 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative levels of - caryophyllene in whole plants in the panicle-formation stage and panicles in the flowering stage were much higher than that in stems and leaves in the flowering stage .
	manualset3
132125	8	406192	13	NULL	NULL	0	NULL	leaves 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative levels of - caryophyllene in whole plants in the panicle-formation stage and panicles in the flowering stage were much higher than that in stems and leaves in the flowering stage .
	manualset3
132126	9	406192	13	NULL	NULL	0	NULL	flowering stage	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative levels of - caryophyllene in whole plants in the panicle-formation stage and panicles in the flowering stage were much higher than that in stems and leaves in the flowering stage .
	manualset3
132127	1	406193	13	NULL	NULL	NULL	NULL	Relative sensitivity	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Relative sensitivity to estrogens was evaluated by reference to 17 beta-estradiol ( E2 ) calibration curves derived using the recombinant yeast cells , MCF-7 human breast cancer cells , and a prepubertal mouse uterotrophic bioassay .
	manualset3
132128	2	406193	13	NULL	NULL	0	NULL	estrogens	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative sensitivity to estrogens was evaluated by reference to 17 beta-estradiol ( E2 ) calibration curves derived using the recombinant yeast cells , MCF-7 human breast cancer cells , and a prepubertal mouse uterotrophic bioassay .
	manualset3
132129	3	406193	13	NULL	NULL	0	NULL	reference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative sensitivity to estrogens was evaluated by reference to 17 beta-estradiol ( E2 ) calibration curves derived using the recombinant yeast cells , MCF-7 human breast cancer cells , and a prepubertal mouse uterotrophic bioassay .
	manualset3
132130	4	406193	13	NULL	NULL	0	NULL	17 beta-estradiol ( E2 ) calibration curves	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative sensitivity to estrogens was evaluated by reference to 17 beta-estradiol ( E2 ) calibration curves derived using the recombinant yeast cells , MCF-7 human breast cancer cells , and a prepubertal mouse uterotrophic bioassay .
	manualset3
132131	5	406193	13	NULL	NULL	0	NULL	recombinant yeast cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative sensitivity to estrogens was evaluated by reference to 17 beta-estradiol ( E2 ) calibration curves derived using the recombinant yeast cells , MCF-7 human breast cancer cells , and a prepubertal mouse uterotrophic bioassay .
	manualset3
132132	6	406193	13	NULL	NULL	0	NULL	MCF-7 human breast cancer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative sensitivity to estrogens was evaluated by reference to 17 beta-estradiol ( E2 ) calibration curves derived using the recombinant yeast cells , MCF-7 human breast cancer cells , and a prepubertal mouse uterotrophic bioassay .
	manualset3
132133	7	406193	13	NULL	NULL	0	NULL	prepubertal mouse uterotrophic bioassay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative sensitivity to estrogens was evaluated by reference to 17 beta-estradiol ( E2 ) calibration curves derived using the recombinant yeast cells , MCF-7 human breast cancer cells , and a prepubertal mouse uterotrophic bioassay .
	manualset3
132238	1	406194	13	NULL	NULL	0	NULL	AP7	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to AP7 , the number of AP7 .3 or PAC1 .
	manualset3
132239	2	406194	13	NULL	NULL	0	NULL	number	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to AP7 , the number of AP7 .3 or PAC1 .
	manualset3
132240	3	406194	13	NULL	NULL	0	NULL	AP7 .3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to AP7 , the number of AP7 .3 or PAC1 .
	manualset3
132241	4	406194	13	NULL	NULL	0	NULL	PAC1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to AP7 , the number of AP7 .3 or PAC1 .
	manualset3
132242	1	406195	13	NULL	NULL	0	NULL	Cardiac arrhythmia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cardiac arrhythmia during pneumatic dilatation of achalasia of the esophagus ( author 's transl ) ) .
	manualset3
132243	2	406195	13	NULL	NULL	0	NULL	pneumatic dilatation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cardiac arrhythmia during pneumatic dilatation of achalasia of the esophagus ( author 's transl ) ) .
	manualset3
132244	3	406195	13	NULL	NULL	0	NULL	achalasia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cardiac arrhythmia during pneumatic dilatation of achalasia of the esophagus ( author 's transl ) ) .
	manualset3
132245	4	406195	13	NULL	NULL	0	NULL	esophagus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cardiac arrhythmia during pneumatic dilatation of achalasia of the esophagus ( author 's transl ) ) .
	manualset3
132246	5	406195	13	NULL	NULL	0	NULL	author 's	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cardiac arrhythmia during pneumatic dilatation of achalasia of the esophagus ( author 's transl ) ) .
	manualset3
132247	6	406195	13	NULL	NULL	0	NULL	transl	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cardiac arrhythmia during pneumatic dilatation of achalasia of the esophagus ( author 's transl ) ) .
	manualset3
132248	1	406196	13	NULL	NULL	0	NULL	issue	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A more difficult issue is the case where a multiplicity of peptides with multiple amino acid substitutions can be associated with pathology .
	manualset3
132249	2	406196	13	NULL	NULL	NULL	NULL	case 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A more difficult issue is the case where a multiplicity of peptides with multiple amino acid substitutions can be associated with pathology .
	manualset3
132250	3	406196	13	NULL	NULL	0	NULL	multiplicity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A more difficult issue is the case where a multiplicity of peptides with multiple amino acid substitutions can be associated with pathology .
	manualset3
132251	4	406196	13	NULL	NULL	0	NULL	peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	A more difficult issue is the case where a multiplicity of peptides with multiple amino acid substitutions can be associated with pathology .
	manualset3
132252	5	406196	13	NULL	NULL	0	NULL	multiple amino acid substitutions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A more difficult issue is the case where a multiplicity of peptides with multiple amino acid substitutions can be associated with pathology .
	manualset3
132253	6	406196	13	NULL	NULL	0	NULL	pathology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A more difficult issue is the case where a multiplicity of peptides with multiple amino acid substitutions can be associated with pathology .
	manualset3
132254	1	406197	13	NULL	NULL	0	NULL	control strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to control strains , the fpg - derivatives were found to be consistently more sensitive to the lethal effects of UVA , but not far-UV radiation .
	manualset3
132255	2	406197	13	NULL	NULL	0	NULL	fpg - derivatives	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to control strains , the fpg - derivatives were found to be consistently more sensitive to the lethal effects of UVA , but not far-UV radiation .
	manualset3
132256	3	406197	13	NULL	NULL	0	NULL	lethal effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to control strains , the fpg - derivatives were found to be consistently more sensitive to the lethal effects of UVA , but not far-UV radiation .
	manualset3
132257	4	406197	13	NULL	NULL	0	NULL	UVA	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to control strains , the fpg - derivatives were found to be consistently more sensitive to the lethal effects of UVA , but not far-UV radiation .
	manualset3
132258	5	406197	13	NULL	NULL	0	NULL	far-UV radiation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to control strains , the fpg - derivatives were found to be consistently more sensitive to the lethal effects of UVA , but not far-UV radiation .
	manualset3
132304	1	406198	13	NULL	NULL	0	NULL	distraction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to distraction , rumination maintained anxiety in both high and low socially anxious individuals , and maintained unconditional beliefs in high socially anxious individuals .
	manualset3
132305	2	406198	13	NULL	NULL	0	NULL	rumination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to distraction , rumination maintained anxiety in both high and low socially anxious individuals , and maintained unconditional beliefs in high socially anxious individuals .
	manualset3
132306	3	406198	13	NULL	NULL	0	NULL	anxiety	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to distraction , rumination maintained anxiety in both high and low socially anxious individuals , and maintained unconditional beliefs in high socially anxious individuals .
	manualset3
132307	4	406198	13	NULL	NULL	0	NULL	anxious individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to distraction , rumination maintained anxiety in both high and low socially anxious individuals , and maintained unconditional beliefs in high socially anxious individuals .
	manualset3
132308	5	406198	13	NULL	NULL	0	NULL	beliefs	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to distraction , rumination maintained anxiety in both high and low socially anxious individuals , and maintained unconditional beliefs in high socially anxious individuals .
	manualset3
132309	6	406198	13	NULL	NULL	0	NULL	anxious individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to distraction , rumination maintained anxiety in both high and low socially anxious individuals , and maintained unconditional beliefs in high socially anxious individuals .
	manualset3
132310	1	406199	13	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to the activity of the CMV promoter , the human endothelial cell-specific promoters all showed less activity in porcine kidney microvascular endothelial cells than in liver or brain microvascular endothelial cells .
	manualset3
132311	2	406199	13	NULL	NULL	0	NULL	CMV promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to the activity of the CMV promoter , the human endothelial cell-specific promoters all showed less activity in porcine kidney microvascular endothelial cells than in liver or brain microvascular endothelial cells .
	manualset3
132312	3	406199	13	NULL	NULL	0	NULL	human endothelial cell-specific promoters	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to the activity of the CMV promoter , the human endothelial cell-specific promoters all showed less activity in porcine kidney microvascular endothelial cells than in liver or brain microvascular endothelial cells .
	manualset3
132313	4	406199	13	NULL	NULL	0	NULL	activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to the activity of the CMV promoter , the human endothelial cell-specific promoters all showed less activity in porcine kidney microvascular endothelial cells than in liver or brain microvascular endothelial cells .
	manualset3
132314	5	406199	13	NULL	NULL	0	NULL	porcine kidney microvascular endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to the activity of the CMV promoter , the human endothelial cell-specific promoters all showed less activity in porcine kidney microvascular endothelial cells than in liver or brain microvascular endothelial cells .
	manualset3
132315	6	406199	13	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to the activity of the CMV promoter , the human endothelial cell-specific promoters all showed less activity in porcine kidney microvascular endothelial cells than in liver or brain microvascular endothelial cells .
	manualset3
132316	7	406199	13	NULL	NULL	0	NULL	brain microvascular endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to the activity of the CMV promoter , the human endothelial cell-specific promoters all showed less activity in porcine kidney microvascular endothelial cells than in liver or brain microvascular endothelial cells .
	manualset3
132317	1	406200	13	NULL	NULL	0	NULL	survey	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to the first survey , the frequency of reported diabetes increased ( 9.7 vs 5.5 % , p & lt ; 0.02 ) , the frequency of hypertension decreased ( 27.6 vs 21.9 % , p & lt ; 0.001 ) , body mass index increased ( 26.3 vs 25.6 kg.m-2 , p & lt ; 0.001 ) , while the lipid levels did not change ( total cholesterol : 2.25 vs 2.29 g/l ; HDL-cholesterol : 0.51 + / - 0.13 vs 0.53 + / - 0.14 g/l ) .
	manualset3
132318	2	406200	13	NULL	NULL	0	NULL	frequency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to the first survey , the frequency of reported diabetes increased ( 9.7 vs 5.5 % , p & lt ; 0.02 ) , the frequency of hypertension decreased ( 27.6 vs 21.9 % , p & lt ; 0.001 ) , body mass index increased ( 26.3 vs 25.6 kg.m-2 , p & lt ; 0.001 ) , while the lipid levels did not change ( total cholesterol : 2.25 vs 2.29 g/l ; HDL-cholesterol : 0.51 + / - 0.13 vs 0.53 + / - 0.14 g/l ) .
	manualset3
132319	3	406200	13	NULL	NULL	0	NULL	diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to the first survey , the frequency of reported diabetes increased ( 9.7 vs 5.5 % , p & lt ; 0.02 ) , the frequency of hypertension decreased ( 27.6 vs 21.9 % , p & lt ; 0.001 ) , body mass index increased ( 26.3 vs 25.6 kg.m-2 , p & lt ; 0.001 ) , while the lipid levels did not change ( total cholesterol : 2.25 vs 2.29 g/l ; HDL-cholesterol : 0.51 + / - 0.13 vs 0.53 + / - 0.14 g/l ) .
	manualset3
132320	4	406200	13	NULL	NULL	0	NULL	9.7 vs 5.5 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to the first survey , the frequency of reported diabetes increased ( 9.7 vs 5.5 % , p & lt ; 0.02 ) , the frequency of hypertension decreased ( 27.6 vs 21.9 % , p & lt ; 0.001 ) , body mass index increased ( 26.3 vs 25.6 kg.m-2 , p & lt ; 0.001 ) , while the lipid levels did not change ( total cholesterol : 2.25 vs 2.29 g/l ; HDL-cholesterol : 0.51 + / - 0.13 vs 0.53 + / - 0.14 g/l ) .
	manualset3
132321	5	406200	13	NULL	NULL	0	NULL	p & lt ; 0.02	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to the first survey , the frequency of reported diabetes increased ( 9.7 vs 5.5 % , p & lt ; 0.02 ) , the frequency of hypertension decreased ( 27.6 vs 21.9 % , p & lt ; 0.001 ) , body mass index increased ( 26.3 vs 25.6 kg.m-2 , p & lt ; 0.001 ) , while the lipid levels did not change ( total cholesterol : 2.25 vs 2.29 g/l ; HDL-cholesterol : 0.51 + / - 0.13 vs 0.53 + / - 0.14 g/l ) .
	manualset3
132322	6	406200	13	NULL	NULL	0	NULL	frequency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to the first survey , the frequency of reported diabetes increased ( 9.7 vs 5.5 % , p & lt ; 0.02 ) , the frequency of hypertension decreased ( 27.6 vs 21.9 % , p & lt ; 0.001 ) , body mass index increased ( 26.3 vs 25.6 kg.m-2 , p & lt ; 0.001 ) , while the lipid levels did not change ( total cholesterol : 2.25 vs 2.29 g/l ; HDL-cholesterol : 0.51 + / - 0.13 vs 0.53 + / - 0.14 g/l ) .
	manualset3
132323	7	406200	13	NULL	NULL	0	NULL	hypertension 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to the first survey , the frequency of reported diabetes increased ( 9.7 vs 5.5 % , p & lt ; 0.02 ) , the frequency of hypertension decreased ( 27.6 vs 21.9 % , p & lt ; 0.001 ) , body mass index increased ( 26.3 vs 25.6 kg.m-2 , p & lt ; 0.001 ) , while the lipid levels did not change ( total cholesterol : 2.25 vs 2.29 g/l ; HDL-cholesterol : 0.51 + / - 0.13 vs 0.53 + / - 0.14 g/l ) .
	manualset3
132324	8	406200	13	NULL	NULL	0	NULL	27.6 vs 21.9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to the first survey , the frequency of reported diabetes increased ( 9.7 vs 5.5 % , p & lt ; 0.02 ) , the frequency of hypertension decreased ( 27.6 vs 21.9 % , p & lt ; 0.001 ) , body mass index increased ( 26.3 vs 25.6 kg.m-2 , p & lt ; 0.001 ) , while the lipid levels did not change ( total cholesterol : 2.25 vs 2.29 g/l ; HDL-cholesterol : 0.51 + / - 0.13 vs 0.53 + / - 0.14 g/l ) .
	manualset3
132325	9	406200	13	NULL	NULL	0	NULL	p & lt ; 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to the first survey , the frequency of reported diabetes increased ( 9.7 vs 5.5 % , p & lt ; 0.02 ) , the frequency of hypertension decreased ( 27.6 vs 21.9 % , p & lt ; 0.001 ) , body mass index increased ( 26.3 vs 25.6 kg.m-2 , p & lt ; 0.001 ) , while the lipid levels did not change ( total cholesterol : 2.25 vs 2.29 g/l ; HDL-cholesterol : 0.51 + / - 0.13 vs 0.53 + / - 0.14 g/l ) .
	manualset3
132326	10	406200	13	NULL	NULL	0	NULL	body mass index	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to the first survey , the frequency of reported diabetes increased ( 9.7 vs 5.5 % , p & lt ; 0.02 ) , the frequency of hypertension decreased ( 27.6 vs 21.9 % , p & lt ; 0.001 ) , body mass index increased ( 26.3 vs 25.6 kg.m-2 , p & lt ; 0.001 ) , while the lipid levels did not change ( total cholesterol : 2.25 vs 2.29 g/l ; HDL-cholesterol : 0.51 + / - 0.13 vs 0.53 + / - 0.14 g/l ) .
	manualset3
132327	11	406200	13	NULL	NULL	0	NULL	26.3 vs 25.6 kg.m-2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to the first survey , the frequency of reported diabetes increased ( 9.7 vs 5.5 % , p & lt ; 0.02 ) , the frequency of hypertension decreased ( 27.6 vs 21.9 % , p & lt ; 0.001 ) , body mass index increased ( 26.3 vs 25.6 kg.m-2 , p & lt ; 0.001 ) , while the lipid levels did not change ( total cholesterol : 2.25 vs 2.29 g/l ; HDL-cholesterol : 0.51 + / - 0.13 vs 0.53 + / - 0.14 g/l ) .
	manualset3
132328	12	406200	13	NULL	NULL	0	NULL	p & lt ; 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to the first survey , the frequency of reported diabetes increased ( 9.7 vs 5.5 % , p & lt ; 0.02 ) , the frequency of hypertension decreased ( 27.6 vs 21.9 % , p & lt ; 0.001 ) , body mass index increased ( 26.3 vs 25.6 kg.m-2 , p & lt ; 0.001 ) , while the lipid levels did not change ( total cholesterol : 2.25 vs 2.29 g/l ; HDL-cholesterol : 0.51 + / - 0.13 vs 0.53 + / - 0.14 g/l ) .
	manualset3
132329	13	406200	13	NULL	NULL	0	NULL	lipid levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to the first survey , the frequency of reported diabetes increased ( 9.7 vs 5.5 % , p & lt ; 0.02 ) , the frequency of hypertension decreased ( 27.6 vs 21.9 % , p & lt ; 0.001 ) , body mass index increased ( 26.3 vs 25.6 kg.m-2 , p & lt ; 0.001 ) , while the lipid levels did not change ( total cholesterol : 2.25 vs 2.29 g/l ; HDL-cholesterol : 0.51 + / - 0.13 vs 0.53 + / - 0.14 g/l ) .
	manualset3
132330	14	406200	13	NULL	NULL	0	NULL	total cholesterol	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to the first survey , the frequency of reported diabetes increased ( 9.7 vs 5.5 % , p & lt ; 0.02 ) , the frequency of hypertension decreased ( 27.6 vs 21.9 % , p & lt ; 0.001 ) , body mass index increased ( 26.3 vs 25.6 kg.m-2 , p & lt ; 0.001 ) , while the lipid levels did not change ( total cholesterol : 2.25 vs 2.29 g/l ; HDL-cholesterol : 0.51 + / - 0.13 vs 0.53 + / - 0.14 g/l ) .
	manualset3
132331	15	406200	13	NULL	NULL	0	NULL	2.25 vs 2.29 g/l	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to the first survey , the frequency of reported diabetes increased ( 9.7 vs 5.5 % , p & lt ; 0.02 ) , the frequency of hypertension decreased ( 27.6 vs 21.9 % , p & lt ; 0.001 ) , body mass index increased ( 26.3 vs 25.6 kg.m-2 , p & lt ; 0.001 ) , while the lipid levels did not change ( total cholesterol : 2.25 vs 2.29 g/l ; HDL-cholesterol : 0.51 + / - 0.13 vs 0.53 + / - 0.14 g/l ) .
	manualset3
132332	16	406200	13	NULL	NULL	0	NULL	HDL-cholesterol 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to the first survey , the frequency of reported diabetes increased ( 9.7 vs 5.5 % , p & lt ; 0.02 ) , the frequency of hypertension decreased ( 27.6 vs 21.9 % , p & lt ; 0.001 ) , body mass index increased ( 26.3 vs 25.6 kg.m-2 , p & lt ; 0.001 ) , while the lipid levels did not change ( total cholesterol : 2.25 vs 2.29 g/l ; HDL-cholesterol : 0.51 + / - 0.13 vs 0.53 + / - 0.14 g/l ) .
	manualset3
132333	17	406200	13	NULL	NULL	0	NULL	0.51 + / - 0.13 vs 0.53 + / - 0.14 g/l	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to the first survey , the frequency of reported diabetes increased ( 9.7 vs 5.5 % , p & lt ; 0.02 ) , the frequency of hypertension decreased ( 27.6 vs 21.9 % , p & lt ; 0.001 ) , body mass index increased ( 26.3 vs 25.6 kg.m-2 , p & lt ; 0.001 ) , while the lipid levels did not change ( total cholesterol : 2.25 vs 2.29 g/l ; HDL-cholesterol : 0.51 + / - 0.13 vs 0.53 + / - 0.14 g/l ) .
	manualset3
132334	1	406201	13	NULL	NULL	0	NULL	Relaxation dynamics	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Relaxation dynamics of tryptophan in water : A UV fluorescence up-conversion and molecular dynamics study .
	manualset3
132335	2	406201	13	NULL	NULL	0	NULL	tryptophan	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Relaxation dynamics of tryptophan in water : A UV fluorescence up-conversion and molecular dynamics study .
	manualset3
132336	3	406201	13	NULL	NULL	0	NULL	water 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Relaxation dynamics of tryptophan in water : A UV fluorescence up-conversion and molecular dynamics study .
	manualset3
132337	4	406201	13	NULL	NULL	0	NULL	UV fluorescence up-conversion	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Relaxation dynamics of tryptophan in water : A UV fluorescence up-conversion and molecular dynamics study .
	manualset3
132338	5	406201	13	NULL	NULL	0	NULL	molecular dynamics 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Relaxation dynamics of tryptophan in water : A UV fluorescence up-conversion and molecular dynamics study .
	manualset3
134872	6	406201	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Relaxation dynamics of tryptophan in water : A UV fluorescence up-conversion and molecular dynamics study .
	manualset3
132339	1	406202	13	NULL	NULL	0	NULL	Release 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Release from cells and brain slices is stimulated by HA and by phorbol ester , and it is blocked by a metalloprotease inhibitor and by lowering the temperature to 20 degrees C. Blockade of SorLA shedding and treatment of cells with SorLA antisense oligonucleotides lead to a decrease in the rate of cell proliferation .
	manualset3
132340	2	406202	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Release from cells and brain slices is stimulated by HA and by phorbol ester , and it is blocked by a metalloprotease inhibitor and by lowering the temperature to 20 degrees C. Blockade of SorLA shedding and treatment of cells with SorLA antisense oligonucleotides lead to a decrease in the rate of cell proliferation .
	manualset3
132341	3	406202	13	NULL	NULL	0	NULL	brain slices	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Release from cells and brain slices is stimulated by HA and by phorbol ester , and it is blocked by a metalloprotease inhibitor and by lowering the temperature to 20 degrees C. Blockade of SorLA shedding and treatment of cells with SorLA antisense oligonucleotides lead to a decrease in the rate of cell proliferation .
	manualset3
132342	4	406202	13	NULL	NULL	0	NULL	HA	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Release from cells and brain slices is stimulated by HA and by phorbol ester , and it is blocked by a metalloprotease inhibitor and by lowering the temperature to 20 degrees C. Blockade of SorLA shedding and treatment of cells with SorLA antisense oligonucleotides lead to a decrease in the rate of cell proliferation .
	manualset3
132343	5	406202	13	NULL	NULL	0	NULL	phorbol ester	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Release from cells and brain slices is stimulated by HA and by phorbol ester , and it is blocked by a metalloprotease inhibitor and by lowering the temperature to 20 degrees C. Blockade of SorLA shedding and treatment of cells with SorLA antisense oligonucleotides lead to a decrease in the rate of cell proliferation .
	manualset3
132344	6	406202	13	NULL	NULL	0	NULL	metalloprotease inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Release from cells and brain slices is stimulated by HA and by phorbol ester , and it is blocked by a metalloprotease inhibitor and by lowering the temperature to 20 degrees C. Blockade of SorLA shedding and treatment of cells with SorLA antisense oligonucleotides lead to a decrease in the rate of cell proliferation .
	manualset3
132345	7	406202	13	NULL	NULL	0	NULL	temperature	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Release from cells and brain slices is stimulated by HA and by phorbol ester , and it is blocked by a metalloprotease inhibitor and by lowering the temperature to 20 degrees C. Blockade of SorLA shedding and treatment of cells with SorLA antisense oligonucleotides lead to a decrease in the rate of cell proliferation .
	manualset3
132346	8	406202	13	NULL	NULL	0	NULL	20 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Release from cells and brain slices is stimulated by HA and by phorbol ester , and it is blocked by a metalloprotease inhibitor and by lowering the temperature to 20 degrees C. Blockade of SorLA shedding and treatment of cells with SorLA antisense oligonucleotides lead to a decrease in the rate of cell proliferation .
	manualset3
132347	9	406202	13	NULL	NULL	0	NULL	Blockade 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Release from cells and brain slices is stimulated by HA and by phorbol ester , and it is blocked by a metalloprotease inhibitor and by lowering the temperature to 20 degrees C. Blockade of SorLA shedding and treatment of cells with SorLA antisense oligonucleotides lead to a decrease in the rate of cell proliferation .
	manualset3
132348	10	406202	13	NULL	NULL	0	NULL	SorLA 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Release from cells and brain slices is stimulated by HA and by phorbol ester , and it is blocked by a metalloprotease inhibitor and by lowering the temperature to 20 degrees C. Blockade of SorLA shedding and treatment of cells with SorLA antisense oligonucleotides lead to a decrease in the rate of cell proliferation .
	manualset3
132349	11	406202	13	NULL	NULL	0	NULL	treatment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Release from cells and brain slices is stimulated by HA and by phorbol ester , and it is blocked by a metalloprotease inhibitor and by lowering the temperature to 20 degrees C. Blockade of SorLA shedding and treatment of cells with SorLA antisense oligonucleotides lead to a decrease in the rate of cell proliferation .
	manualset3
132350	12	406202	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Release from cells and brain slices is stimulated by HA and by phorbol ester , and it is blocked by a metalloprotease inhibitor and by lowering the temperature to 20 degrees C. Blockade of SorLA shedding and treatment of cells with SorLA antisense oligonucleotides lead to a decrease in the rate of cell proliferation .
	manualset3
132351	13	406202	13	NULL	NULL	0	NULL	SorLA antisense oligonucleotides 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Release from cells and brain slices is stimulated by HA and by phorbol ester , and it is blocked by a metalloprotease inhibitor and by lowering the temperature to 20 degrees C. Blockade of SorLA shedding and treatment of cells with SorLA antisense oligonucleotides lead to a decrease in the rate of cell proliferation .
	manualset3
132352	14	406202	13	NULL	NULL	0	NULL	decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Release from cells and brain slices is stimulated by HA and by phorbol ester , and it is blocked by a metalloprotease inhibitor and by lowering the temperature to 20 degrees C. Blockade of SorLA shedding and treatment of cells with SorLA antisense oligonucleotides lead to a decrease in the rate of cell proliferation .
	manualset3
132353	15	406202	13	NULL	NULL	0	NULL	rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Release from cells and brain slices is stimulated by HA and by phorbol ester , and it is blocked by a metalloprotease inhibitor and by lowering the temperature to 20 degrees C. Blockade of SorLA shedding and treatment of cells with SorLA antisense oligonucleotides lead to a decrease in the rate of cell proliferation .
	manualset3
132354	16	406202	13	NULL	NULL	0	NULL	cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Release from cells and brain slices is stimulated by HA and by phorbol ester , and it is blocked by a metalloprotease inhibitor and by lowering the temperature to 20 degrees C. Blockade of SorLA shedding and treatment of cells with SorLA antisense oligonucleotides lead to a decrease in the rate of cell proliferation .
	manualset3
132355	1	406203	13	NULL	NULL	0	NULL	Release 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Release of glutamate and influx of Ca2 + are the most important triggering factors .
	manualset3
132356	2	406203	13	NULL	NULL	0	NULL	glutamate	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Release of glutamate and influx of Ca2 + are the most important triggering factors .
	manualset3
132357	3	406203	13	NULL	NULL	0	NULL	influx	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Release of glutamate and influx of Ca2 + are the most important triggering factors .
	manualset3
132358	4	406203	13	NULL	NULL	0	NULL	Ca2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Release of glutamate and influx of Ca2 + are the most important triggering factors .
	manualset3
132359	5	406203	13	NULL	NULL	0	NULL	triggering factors	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Release of glutamate and influx of Ca2 + are the most important triggering factors .
	manualset3
132360	1	406204	13	NULL	NULL	0	NULL	intensive vasoconstrictive response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A more intensive vasoconstrictive response in perfusion with a constant discharge was observed in spontaneously hypertensive rats as compared to normotensive ones , and in perfusion with a constant pressure the reverse correlation was noted .
	manualset3
132361	2	406204	13	NULL	NULL	0	NULL	perfusion 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A more intensive vasoconstrictive response in perfusion with a constant discharge was observed in spontaneously hypertensive rats as compared to normotensive ones , and in perfusion with a constant pressure the reverse correlation was noted .
	manualset3
132362	3	406204	13	NULL	NULL	0	NULL	discharge 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A more intensive vasoconstrictive response in perfusion with a constant discharge was observed in spontaneously hypertensive rats as compared to normotensive ones , and in perfusion with a constant pressure the reverse correlation was noted .
	manualset3
132363	4	406204	13	NULL	NULL	0	NULL	hypertensive rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A more intensive vasoconstrictive response in perfusion with a constant discharge was observed in spontaneously hypertensive rats as compared to normotensive ones , and in perfusion with a constant pressure the reverse correlation was noted .
	manualset3
132364	5	406204	13	NULL	NULL	0	NULL	normotensive ones	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A more intensive vasoconstrictive response in perfusion with a constant discharge was observed in spontaneously hypertensive rats as compared to normotensive ones , and in perfusion with a constant pressure the reverse correlation was noted .
	manualset3
132365	6	406204	13	NULL	NULL	0	NULL	perfusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A more intensive vasoconstrictive response in perfusion with a constant discharge was observed in spontaneously hypertensive rats as compared to normotensive ones , and in perfusion with a constant pressure the reverse correlation was noted .
	manualset3
132366	7	406204	13	NULL	NULL	0	NULL	pressure 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A more intensive vasoconstrictive response in perfusion with a constant discharge was observed in spontaneously hypertensive rats as compared to normotensive ones , and in perfusion with a constant pressure the reverse correlation was noted .
	manualset3
132367	8	406204	13	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A more intensive vasoconstrictive response in perfusion with a constant discharge was observed in spontaneously hypertensive rats as compared to normotensive ones , and in perfusion with a constant pressure the reverse correlation was noted .
	manualset3
132368	1	406205	13	NULL	NULL	0	NULL	Release studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Release studies have shown that the stability of Egg-PC/PEG ( 45 ) - Tetraether-based archaeosomes is significantly higher at 37C than the one of Egg-PC/PEG ( 45 ) - DSPE-based liposomes , as evidenced by the slower release of the dye encapsulated into PEGylated archaeosomes .
	manualset3
132369	2	406205	13	NULL	NULL	0	NULL	stability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Release studies have shown that the stability of Egg-PC/PEG ( 45 ) - Tetraether-based archaeosomes is significantly higher at 37C than the one of Egg-PC/PEG ( 45 ) - DSPE-based liposomes , as evidenced by the slower release of the dye encapsulated into PEGylated archaeosomes .
	manualset3
132370	3	406205	13	NULL	NULL	0	NULL	Egg-PC/PEG ( 45 ) - Tetraether-based archaeosomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Release studies have shown that the stability of Egg-PC/PEG ( 45 ) - Tetraether-based archaeosomes is significantly higher at 37C than the one of Egg-PC/PEG ( 45 ) - DSPE-based liposomes , as evidenced by the slower release of the dye encapsulated into PEGylated archaeosomes .
	manualset3
132371	4	406205	13	NULL	NULL	0	NULL	37C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Release studies have shown that the stability of Egg-PC/PEG ( 45 ) - Tetraether-based archaeosomes is significantly higher at 37C than the one of Egg-PC/PEG ( 45 ) - DSPE-based liposomes , as evidenced by the slower release of the dye encapsulated into PEGylated archaeosomes .
	manualset3
132372	5	406205	13	NULL	NULL	0	NULL	Egg-PC/PEG ( 45 ) - DSPE-based liposomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Release studies have shown that the stability of Egg-PC/PEG ( 45 ) - Tetraether-based archaeosomes is significantly higher at 37C than the one of Egg-PC/PEG ( 45 ) - DSPE-based liposomes , as evidenced by the slower release of the dye encapsulated into PEGylated archaeosomes .
	manualset3
132373	6	406205	13	NULL	NULL	0	NULL	release	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Release studies have shown that the stability of Egg-PC/PEG ( 45 ) - Tetraether-based archaeosomes is significantly higher at 37C than the one of Egg-PC/PEG ( 45 ) - DSPE-based liposomes , as evidenced by the slower release of the dye encapsulated into PEGylated archaeosomes .
	manualset3
132374	7	406205	13	NULL	NULL	0	NULL	dye	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Release studies have shown that the stability of Egg-PC/PEG ( 45 ) - Tetraether-based archaeosomes is significantly higher at 37C than the one of Egg-PC/PEG ( 45 ) - DSPE-based liposomes , as evidenced by the slower release of the dye encapsulated into PEGylated archaeosomes .
	manualset3
132375	8	406205	13	NULL	NULL	0	NULL	PEGylated archaeosomes 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Release studies have shown that the stability of Egg-PC/PEG ( 45 ) - Tetraether-based archaeosomes is significantly higher at 37C than the one of Egg-PC/PEG ( 45 ) - DSPE-based liposomes , as evidenced by the slower release of the dye encapsulated into PEGylated archaeosomes .
	manualset3
132376	1	406206	13	NULL	NULL	0	NULL	Religious influences	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Religious influences on heavy episodic drinking in Chinese-American and Korean-American college students .
	manualset3
132377	2	406206	13	NULL	NULL	0	NULL	Chinese-American college students	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Religious influences on heavy episodic drinking in Chinese-American and Korean-American college students .
	manualset3
132378	3	406206	13	NULL	NULL	0	NULL	Korean-American college students	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Religious influences on heavy episodic drinking in Chinese-American and Korean-American college students .
	manualset3
134885	4	406206	13	NULL	NULL	0	NULL	episodic drinking	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Religious influences on heavy episodic drinking in Chinese-American and Korean-American college students .
	manualset3
132379	1	406207	13	NULL	NULL	0	NULL	correlations 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Remaining significant correlations were between auditory short term memory and all other included measures , expressive language and all other included measures , and CA and auditory short term memory and expressive language .
	manualset3
132380	2	406207	13	NULL	NULL	0	NULL	auditory short term memory	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Remaining significant correlations were between auditory short term memory and all other included measures , expressive language and all other included measures , and CA and auditory short term memory and expressive language .
	manualset3
132381	3	406207	13	NULL	NULL	0	NULL	measures 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Remaining significant correlations were between auditory short term memory and all other included measures , expressive language and all other included measures , and CA and auditory short term memory and expressive language .
	manualset3
132382	4	406207	13	NULL	NULL	0	NULL	expressive language	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Remaining significant correlations were between auditory short term memory and all other included measures , expressive language and all other included measures , and CA and auditory short term memory and expressive language .
	manualset3
132383	5	406207	13	NULL	NULL	0	NULL	measures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Remaining significant correlations were between auditory short term memory and all other included measures , expressive language and all other included measures , and CA and auditory short term memory and expressive language .
	manualset3
132384	6	406207	13	NULL	NULL	0	NULL	CA	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Remaining significant correlations were between auditory short term memory and all other included measures , expressive language and all other included measures , and CA and auditory short term memory and expressive language .
	manualset3
132385	7	406207	13	NULL	NULL	0	NULL	auditory short term memory 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Remaining significant correlations were between auditory short term memory and all other included measures , expressive language and all other included measures , and CA and auditory short term memory and expressive language .
	manualset3
132386	8	406207	13	NULL	NULL	0	NULL	expressive language	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Remaining significant correlations were between auditory short term memory and all other included measures , expressive language and all other included measures , and CA and auditory short term memory and expressive language .
	manualset3
132387	1	406208	13	NULL	NULL	0	NULL	Dpl-programmed ataxia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably , Dpl-programmed ataxia is rescued by wild-type Prnp transgenes .
	manualset3
132388	2	406208	13	NULL	NULL	0	NULL	wild-type Prnp transgenes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably , Dpl-programmed ataxia is rescued by wild-type Prnp transgenes .
	manualset3
132389	1	406209	13	NULL	NULL	0	NULL	permutation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably , this infrequently occurring permutation was for the first time observed in the periplasmic domain of EpsM ( peri-EpsM ) , another T2SS protein which interacts with EpsL .
	manualset3
132390	2	406209	13	NULL	NULL	NULL	NULL	periplasmic domain of EpsM ( peri-EpsM )	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Remarkably , this infrequently occurring permutation was for the first time observed in the periplasmic domain of EpsM ( peri-EpsM ) , another T2SS protein which interacts with EpsL .
	manualset3
132391	3	406209	13	NULL	NULL	0	NULL	T2SS protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably , this infrequently occurring permutation was for the first time observed in the periplasmic domain of EpsM ( peri-EpsM ) , another T2SS protein which interacts with EpsL .
	manualset3
132392	4	406209	13	NULL	NULL	0	NULL	EpsL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably , this infrequently occurring permutation was for the first time observed in the periplasmic domain of EpsM ( peri-EpsM ) , another T2SS protein which interacts with EpsL .
	manualset3
134886	5	406209	13	NULL	NULL	0	NULL	first time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably , this infrequently occurring permutation was for the first time observed in the periplasmic domain of EpsM ( peri-EpsM ) , another T2SS protein which interacts with EpsL .
	manualset3
132393	1	406210	13	NULL	NULL	0	NULL	levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably higher levels of productivity ( 1.66-1 .84 g l ( -1 ) h ( -1 ) ) was obtained during first five cycles of fermentation with a maximum productivity ( 1.84 g l ( -1 ) h ( -1 ) ) obtained during third cycle of fermentation .
	manualset3
132394	2	406210	13	NULL	NULL	0	NULL	productivity 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably higher levels of productivity ( 1.66-1 .84 g l ( -1 ) h ( -1 ) ) was obtained during first five cycles of fermentation with a maximum productivity ( 1.84 g l ( -1 ) h ( -1 ) ) obtained during third cycle of fermentation .
	manualset3
132395	3	406210	13	NULL	NULL	0	NULL	1.66-1 .84 g l ( -1 ) h ( -1 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably higher levels of productivity ( 1.66-1 .84 g l ( -1 ) h ( -1 ) ) was obtained during first five cycles of fermentation with a maximum productivity ( 1.84 g l ( -1 ) h ( -1 ) ) obtained during third cycle of fermentation .
	manualset3
132396	4	406210	13	NULL	NULL	0	NULL	five cycles 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably higher levels of productivity ( 1.66-1 .84 g l ( -1 ) h ( -1 ) ) was obtained during first five cycles of fermentation with a maximum productivity ( 1.84 g l ( -1 ) h ( -1 ) ) obtained during third cycle of fermentation .
	manualset3
132397	5	406210	13	NULL	NULL	0	NULL	fermentation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably higher levels of productivity ( 1.66-1 .84 g l ( -1 ) h ( -1 ) ) was obtained during first five cycles of fermentation with a maximum productivity ( 1.84 g l ( -1 ) h ( -1 ) ) obtained during third cycle of fermentation .
	manualset3
132398	6	406210	13	NULL	NULL	0	NULL	productivity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably higher levels of productivity ( 1.66-1 .84 g l ( -1 ) h ( -1 ) ) was obtained during first five cycles of fermentation with a maximum productivity ( 1.84 g l ( -1 ) h ( -1 ) ) obtained during third cycle of fermentation .
	manualset3
132399	7	406210	13	NULL	NULL	0	NULL	1.84 g l ( -1 ) h ( -1 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably higher levels of productivity ( 1.66-1 .84 g l ( -1 ) h ( -1 ) ) was obtained during first five cycles of fermentation with a maximum productivity ( 1.84 g l ( -1 ) h ( -1 ) ) obtained during third cycle of fermentation .
	manualset3
132400	8	406210	13	NULL	NULL	0	NULL	third cycle	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably higher levels of productivity ( 1.66-1 .84 g l ( -1 ) h ( -1 ) ) was obtained during first five cycles of fermentation with a maximum productivity ( 1.84 g l ( -1 ) h ( -1 ) ) obtained during third cycle of fermentation .
	manualset3
132401	9	406210	13	NULL	NULL	0	NULL	fermentation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably higher levels of productivity ( 1.66-1 .84 g l ( -1 ) h ( -1 ) ) was obtained during first five cycles of fermentation with a maximum productivity ( 1.84 g l ( -1 ) h ( -1 ) ) obtained during third cycle of fermentation .
	manualset3
132402	1	406211	13	NULL	NULL	0	NULL	Remarks	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarks on the Treatment of the Pyrexia of Phthisis .
	manualset3
132403	2	406211	13	NULL	NULL	0	NULL	Treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarks on the Treatment of the Pyrexia of Phthisis .
	manualset3
132404	3	406211	13	NULL	NULL	0	NULL	Pyrexia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarks on the Treatment of the Pyrexia of Phthisis .
	manualset3
132405	4	406211	13	NULL	NULL	0	NULL	Phthisis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarks on the Treatment of the Pyrexia of Phthisis .
	manualset3
132406	1	406212	13	NULL	NULL	0	NULL	Reminiscences	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reminiscences of a child neurologist .
	manualset3
132407	2	406212	13	NULL	NULL	0	NULL	child neurologist	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Reminiscences of a child neurologist .
	manualset3
132408	1	406213	13	NULL	NULL	0	NULL	accumulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A more rapid accumulation of H + during intense stimulation may lead to a earlier onset of fatigue in the aged muscle .
	manualset3
132409	2	406213	13	NULL	NULL	0	NULL	H + 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	A more rapid accumulation of H + during intense stimulation may lead to a earlier onset of fatigue in the aged muscle .
	manualset3
132410	3	406213	13	NULL	NULL	0	NULL	intense stimulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A more rapid accumulation of H + during intense stimulation may lead to a earlier onset of fatigue in the aged muscle .
	manualset3
132411	4	406213	13	NULL	NULL	0	NULL	onset of fatigue	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A more rapid accumulation of H + during intense stimulation may lead to a earlier onset of fatigue in the aged muscle .
	manualset3
132412	5	406213	13	NULL	NULL	0	NULL	aged muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A more rapid accumulation of H + during intense stimulation may lead to a earlier onset of fatigue in the aged muscle .
	manualset3
132413	1	406214	13	NULL	NULL	0	NULL	functionalisation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Remote functionalisation via sodium alkylamidozincate intermediates : access to unusual fluorenone and pyridyl ketone reactivity patterns .
	manualset3
132414	2	406214	13	NULL	NULL	0	NULL	sodium alkylamidozincate intermediates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Remote functionalisation via sodium alkylamidozincate intermediates : access to unusual fluorenone and pyridyl ketone reactivity patterns .
	manualset3
132415	3	406214	13	NULL	NULL	0	NULL	access	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Remote functionalisation via sodium alkylamidozincate intermediates : access to unusual fluorenone and pyridyl ketone reactivity patterns .
	manualset3
132416	4	406214	13	NULL	NULL	0	NULL	fluorenone reactivity patterns	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Remote functionalisation via sodium alkylamidozincate intermediates : access to unusual fluorenone and pyridyl ketone reactivity patterns .
	manualset3
132417	5	406214	13	NULL	NULL	0	NULL	pyridyl ketone reactivity patterns	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Remote functionalisation via sodium alkylamidozincate intermediates : access to unusual fluorenone and pyridyl ketone reactivity patterns .
	manualset3
132418	1	406215	13	NULL	NULL	0	NULL	Remote sensing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Remote sensing provides an overview of environmental complexities in the Mediterranean region , relating to its natural setting and to water exchanges within the basin ; to typical ecological processes and their key driving forces ; to environmental problems faced by the main sub-basins .
	manualset3
132419	2	406215	13	NULL	NULL	0	NULL	overview	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Remote sensing provides an overview of environmental complexities in the Mediterranean region , relating to its natural setting and to water exchanges within the basin ; to typical ecological processes and their key driving forces ; to environmental problems faced by the main sub-basins .
	manualset3
132420	3	406215	13	NULL	NULL	0	NULL	environmental complexities	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Remote sensing provides an overview of environmental complexities in the Mediterranean region , relating to its natural setting and to water exchanges within the basin ; to typical ecological processes and their key driving forces ; to environmental problems faced by the main sub-basins .
	manualset3
132421	4	406215	13	NULL	NULL	0	NULL	Mediterranean region	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Remote sensing provides an overview of environmental complexities in the Mediterranean region , relating to its natural setting and to water exchanges within the basin ; to typical ecological processes and their key driving forces ; to environmental problems faced by the main sub-basins .
	manualset3
132422	5	406215	13	NULL	NULL	0	NULL	natural setting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Remote sensing provides an overview of environmental complexities in the Mediterranean region , relating to its natural setting and to water exchanges within the basin ; to typical ecological processes and their key driving forces ; to environmental problems faced by the main sub-basins .
	manualset3
132423	6	406215	13	NULL	NULL	0	NULL	water exchanges 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Remote sensing provides an overview of environmental complexities in the Mediterranean region , relating to its natural setting and to water exchanges within the basin ; to typical ecological processes and their key driving forces ; to environmental problems faced by the main sub-basins .
	manualset3
132424	7	406215	13	NULL	NULL	0	NULL	basin	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Remote sensing provides an overview of environmental complexities in the Mediterranean region , relating to its natural setting and to water exchanges within the basin ; to typical ecological processes and their key driving forces ; to environmental problems faced by the main sub-basins .
	manualset3
132425	8	406215	13	NULL	NULL	0	NULL	ecological processes	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Remote sensing provides an overview of environmental complexities in the Mediterranean region , relating to its natural setting and to water exchanges within the basin ; to typical ecological processes and their key driving forces ; to environmental problems faced by the main sub-basins .
	manualset3
132426	9	406215	13	NULL	NULL	0	NULL	key driving forces	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Remote sensing provides an overview of environmental complexities in the Mediterranean region , relating to its natural setting and to water exchanges within the basin ; to typical ecological processes and their key driving forces ; to environmental problems faced by the main sub-basins .
	manualset3
132427	10	406215	13	NULL	NULL	0	NULL	environmental problems	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Remote sensing provides an overview of environmental complexities in the Mediterranean region , relating to its natural setting and to water exchanges within the basin ; to typical ecological processes and their key driving forces ; to environmental problems faced by the main sub-basins .
	manualset3
132428	11	406215	13	NULL	NULL	0	NULL	sub-basins	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Remote sensing provides an overview of environmental complexities in the Mediterranean region , relating to its natural setting and to water exchanges within the basin ; to typical ecological processes and their key driving forces ; to environmental problems faced by the main sub-basins .
	manualset3
132429	1	406216	13	NULL	NULL	0	NULL	Removal 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of basic dye by modified Unye bentonite , Turkey .
	manualset3
132430	2	406216	13	NULL	NULL	0	NULL	basic dye 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of basic dye by modified Unye bentonite , Turkey .
	manualset3
132431	3	406216	13	NULL	NULL	0	NULL	Unye bentonite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of basic dye by modified Unye bentonite , Turkey .
	manualset3
132432	4	406216	13	NULL	NULL	0	NULL	Turkey 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of basic dye by modified Unye bentonite , Turkey .
	manualset3
132433	1	406217	13	NULL	NULL	0	NULL	Removal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of calcium as well as magnesium from the perfusion solution causes a rapid loss of tension in the electrically driven frog ventricle ( 0.4 ) Hz .
	manualset3
132434	2	406217	13	NULL	NULL	0	NULL	calcium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of calcium as well as magnesium from the perfusion solution causes a rapid loss of tension in the electrically driven frog ventricle ( 0.4 ) Hz .
	manualset3
132435	3	406217	13	NULL	NULL	0	NULL	magnesium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of calcium as well as magnesium from the perfusion solution causes a rapid loss of tension in the electrically driven frog ventricle ( 0.4 ) Hz .
	manualset3
132436	4	406217	13	NULL	NULL	0	NULL	perfusion solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of calcium as well as magnesium from the perfusion solution causes a rapid loss of tension in the electrically driven frog ventricle ( 0.4 ) Hz .
	manualset3
132437	5	406217	13	NULL	NULL	0	NULL	loss of tension 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of calcium as well as magnesium from the perfusion solution causes a rapid loss of tension in the electrically driven frog ventricle ( 0.4 ) Hz .
	manualset3
132438	6	406217	13	NULL	NULL	0	NULL	frog ventricle 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of calcium as well as magnesium from the perfusion solution causes a rapid loss of tension in the electrically driven frog ventricle ( 0.4 ) Hz .
	manualset3
132439	7	406217	13	NULL	NULL	0	NULL	( 0.4 ) Hz	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of calcium as well as magnesium from the perfusion solution causes a rapid loss of tension in the electrically driven frog ventricle ( 0.4 ) Hz .
	manualset3
132440	1	406218	13	NULL	NULL	0	NULL	Removal  	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of culturable FC was the most efficient in treatments with high retention time ( activated sludge process with nitrification and denitrification , lagooning ) , in biofiltration and in the treatment with a tertiary disinfection step .
	manualset3
132441	2	406218	13	NULL	NULL	0	NULL	culturable FC	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of culturable FC was the most efficient in treatments with high retention time ( activated sludge process with nitrification and denitrification , lagooning ) , in biofiltration and in the treatment with a tertiary disinfection step .
	manualset3
132442	3	406218	13	NULL	NULL	NULL	NULL	treatments	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Removal of culturable FC was the most efficient in treatments with high retention time ( activated sludge process with nitrification and denitrification , lagooning ) , in biofiltration and in the treatment with a tertiary disinfection step .
	manualset3
132443	4	406218	13	NULL	NULL	0	NULL	retention time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of culturable FC was the most efficient in treatments with high retention time ( activated sludge process with nitrification and denitrification , lagooning ) , in biofiltration and in the treatment with a tertiary disinfection step .
	manualset3
132444	5	406218	13	NULL	NULL	0	NULL	sludge process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of culturable FC was the most efficient in treatments with high retention time ( activated sludge process with nitrification and denitrification , lagooning ) , in biofiltration and in the treatment with a tertiary disinfection step .
	manualset3
132445	6	406218	13	NULL	NULL	0	NULL	nitrification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of culturable FC was the most efficient in treatments with high retention time ( activated sludge process with nitrification and denitrification , lagooning ) , in biofiltration and in the treatment with a tertiary disinfection step .
	manualset3
132446	7	406218	13	NULL	NULL	0	NULL	denitrification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of culturable FC was the most efficient in treatments with high retention time ( activated sludge process with nitrification and denitrification , lagooning ) , in biofiltration and in the treatment with a tertiary disinfection step .
	manualset3
132447	8	406218	13	NULL	NULL	0	NULL	biofiltration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of culturable FC was the most efficient in treatments with high retention time ( activated sludge process with nitrification and denitrification , lagooning ) , in biofiltration and in the treatment with a tertiary disinfection step .
	manualset3
132448	9	406218	13	NULL	NULL	0	NULL	treatment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of culturable FC was the most efficient in treatments with high retention time ( activated sludge process with nitrification and denitrification , lagooning ) , in biofiltration and in the treatment with a tertiary disinfection step .
	manualset3
132449	10	406218	13	NULL	NULL	0	NULL	tertiary disinfection step	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of culturable FC was the most efficient in treatments with high retention time ( activated sludge process with nitrification and denitrification , lagooning ) , in biofiltration and in the treatment with a tertiary disinfection step .
	manualset3
134888	11	406218	13	NULL	NULL	0	NULL	lagooning 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of culturable FC was the most efficient in treatments with high retention time ( activated sludge process with nitrification and denitrification , lagooning ) , in biofiltration and in the treatment with a tertiary disinfection step .
	manualset3
132450	1	406219	13	NULL	NULL	0	NULL	Removal 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of epithelial cells from human intestine explants reduced cholesterol , but not sitosterol , uptake .
	manualset3
132451	2	406219	13	NULL	NULL	0	NULL	epithelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of epithelial cells from human intestine explants reduced cholesterol , but not sitosterol , uptake .
	manualset3
132452	3	406219	13	NULL	NULL	0	NULL	human intestine explants	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of epithelial cells from human intestine explants reduced cholesterol , but not sitosterol , uptake .
	manualset3
132453	4	406219	13	NULL	NULL	0	NULL	cholesterol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of epithelial cells from human intestine explants reduced cholesterol , but not sitosterol , uptake .
	manualset3
132454	5	406219	13	NULL	NULL	0	NULL	sitosterol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of epithelial cells from human intestine explants reduced cholesterol , but not sitosterol , uptake .
	manualset3
132455	6	406219	13	NULL	NULL	0	NULL	uptake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of epithelial cells from human intestine explants reduced cholesterol , but not sitosterol , uptake .
	manualset3
132456	1	406220	13	NULL	NULL	0	NULL	Removal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of the GPE-rosetting cells ( GPE-1 and/or GPE-2 ) from PBL led to a marked decrease in Con A-induced IL-2 synthesis while removal of the GE-rosetting cells yielded a normal or slightly greater than normal response .
	manualset3
132457	2	406220	13	NULL	NULL	0	NULL	GPE-rosetting cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of the GPE-rosetting cells ( GPE-1 and/or GPE-2 ) from PBL led to a marked decrease in Con A-induced IL-2 synthesis while removal of the GE-rosetting cells yielded a normal or slightly greater than normal response .
	manualset3
132458	3	406220	13	NULL	NULL	0	NULL	GPE-1	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of the GPE-rosetting cells ( GPE-1 and/or GPE-2 ) from PBL led to a marked decrease in Con A-induced IL-2 synthesis while removal of the GE-rosetting cells yielded a normal or slightly greater than normal response .
	manualset3
132459	4	406220	13	NULL	NULL	0	NULL	GPE-2	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of the GPE-rosetting cells ( GPE-1 and/or GPE-2 ) from PBL led to a marked decrease in Con A-induced IL-2 synthesis while removal of the GE-rosetting cells yielded a normal or slightly greater than normal response .
	manualset3
132460	5	406220	13	NULL	NULL	0	NULL	PBL 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of the GPE-rosetting cells ( GPE-1 and/or GPE-2 ) from PBL led to a marked decrease in Con A-induced IL-2 synthesis while removal of the GE-rosetting cells yielded a normal or slightly greater than normal response .
	manualset3
132461	6	406220	13	NULL	NULL	0	NULL	decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of the GPE-rosetting cells ( GPE-1 and/or GPE-2 ) from PBL led to a marked decrease in Con A-induced IL-2 synthesis while removal of the GE-rosetting cells yielded a normal or slightly greater than normal response .
	manualset3
132462	7	406220	13	NULL	NULL	0	NULL	Con A-induced IL-2 synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of the GPE-rosetting cells ( GPE-1 and/or GPE-2 ) from PBL led to a marked decrease in Con A-induced IL-2 synthesis while removal of the GE-rosetting cells yielded a normal or slightly greater than normal response .
	manualset3
132463	8	406220	13	NULL	NULL	0	NULL	removal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of the GPE-rosetting cells ( GPE-1 and/or GPE-2 ) from PBL led to a marked decrease in Con A-induced IL-2 synthesis while removal of the GE-rosetting cells yielded a normal or slightly greater than normal response .
	manualset3
132464	9	406220	13	NULL	NULL	0	NULL	GE-rosetting cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of the GPE-rosetting cells ( GPE-1 and/or GPE-2 ) from PBL led to a marked decrease in Con A-induced IL-2 synthesis while removal of the GE-rosetting cells yielded a normal or slightly greater than normal response .
	manualset3
132465	10	406220	13	NULL	NULL	NULL	NULL	response 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Removal of the GPE-rosetting cells ( GPE-1 and/or GPE-2 ) from PBL led to a marked decrease in Con A-induced IL-2 synthesis while removal of the GE-rosetting cells yielded a normal or slightly greater than normal response .
	manualset3
132466	1	406221	13	NULL	NULL	0	NULL	Renal Cd level 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal Cd level observed at 4 h increased with dose , but the Cd concentration in the supernatant fraction was kept almost constant at higher doses .
	manualset3
132467	2	406221	13	NULL	NULL	0	NULL	4 h 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal Cd level observed at 4 h increased with dose , but the Cd concentration in the supernatant fraction was kept almost constant at higher doses .
	manualset3
132468	3	406221	13	NULL	NULL	0	NULL	dose 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal Cd level observed at 4 h increased with dose , but the Cd concentration in the supernatant fraction was kept almost constant at higher doses .
	manualset3
132469	4	406221	13	NULL	NULL	0	NULL	Cd concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal Cd level observed at 4 h increased with dose , but the Cd concentration in the supernatant fraction was kept almost constant at higher doses .
	manualset3
132470	5	406221	13	NULL	NULL	0	NULL	supernatant fraction	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal Cd level observed at 4 h increased with dose , but the Cd concentration in the supernatant fraction was kept almost constant at higher doses .
	manualset3
132471	6	406221	13	NULL	NULL	0	NULL	doses	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal Cd level observed at 4 h increased with dose , but the Cd concentration in the supernatant fraction was kept almost constant at higher doses .
	manualset3
132472	1	406222	13	NULL	NULL	0	NULL	Renal blood flow velocity waveforms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal blood flow velocity waveforms were recorded by Doppler ultrasonography in 114 growth-retarded fetuses and in 97 post-term fetuses .
	manualset3
132473	2	406222	13	NULL	NULL	0	NULL	Doppler ultrasonography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal blood flow velocity waveforms were recorded by Doppler ultrasonography in 114 growth-retarded fetuses and in 97 post-term fetuses .
	manualset3
132474	3	406222	13	NULL	NULL	0	NULL	114 growth-retarded fetuses	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal blood flow velocity waveforms were recorded by Doppler ultrasonography in 114 growth-retarded fetuses and in 97 post-term fetuses .
	manualset3
132475	4	406222	13	NULL	NULL	0	NULL	97 post-term fetuses 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal blood flow velocity waveforms were recorded by Doppler ultrasonography in 114 growth-retarded fetuses and in 97 post-term fetuses .
	manualset3
132476	1	406223	13	NULL	NULL	0	NULL	Renal clearance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal clearance of endogenous creatinine , urea , sodium , and potassium in normal cats and cats with chronic renal failure .
	manualset3
132477	2	406223	13	NULL	NULL	0	NULL	endogenous creatinine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal clearance of endogenous creatinine , urea , sodium , and potassium in normal cats and cats with chronic renal failure .
	manualset3
132478	3	406223	13	NULL	NULL	0	NULL	urea 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal clearance of endogenous creatinine , urea , sodium , and potassium in normal cats and cats with chronic renal failure .
	manualset3
132479	4	406223	13	NULL	NULL	NULL	NULL	sodium	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Renal clearance of endogenous creatinine , urea , sodium , and potassium in normal cats and cats with chronic renal failure .
	manualset3
132480	5	406223	13	NULL	NULL	0	NULL	potassium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal clearance of endogenous creatinine , urea , sodium , and potassium in normal cats and cats with chronic renal failure .
	manualset3
132481	6	406223	13	NULL	NULL	0	NULL	cats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal clearance of endogenous creatinine , urea , sodium , and potassium in normal cats and cats with chronic renal failure .
	manualset3
132482	7	406223	13	NULL	NULL	0	NULL	cats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal clearance of endogenous creatinine , urea , sodium , and potassium in normal cats and cats with chronic renal failure .
	manualset3
132483	8	406223	13	NULL	NULL	0	NULL	chronic renal failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal clearance of endogenous creatinine , urea , sodium , and potassium in normal cats and cats with chronic renal failure .
	manualset3
132484	1	406224	13	NULL	NULL	0	NULL	Renal fibrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal fibrosis is a complication of kidney injury and can contribute to organ failure .
	manualset3
132485	2	406224	13	NULL	NULL	0	NULL	complication 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal fibrosis is a complication of kidney injury and can contribute to organ failure .
	manualset3
132486	3	406224	13	NULL	NULL	0	NULL	kidney injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal fibrosis is a complication of kidney injury and can contribute to organ failure .
	manualset3
132487	4	406224	13	NULL	NULL	0	NULL	organ failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal fibrosis is a complication of kidney injury and can contribute to organ failure .
	manualset3
132488	1	406225	13	NULL	NULL	0	NULL	Renal function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal function after partial nephrectomy : effect of warm ischemia relative to quantity and quality of preserved kidney .
	manualset3
132489	2	406225	13	NULL	NULL	0	NULL	partial nephrectomy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal function after partial nephrectomy : effect of warm ischemia relative to quantity and quality of preserved kidney .
	manualset3
132490	3	406225	13	NULL	NULL	0	NULL	effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal function after partial nephrectomy : effect of warm ischemia relative to quantity and quality of preserved kidney .
	manualset3
132491	4	406225	13	NULL	NULL	0	NULL	warm ischemia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal function after partial nephrectomy : effect of warm ischemia relative to quantity and quality of preserved kidney .
	manualset3
132492	5	406225	13	NULL	NULL	0	NULL	quantity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal function after partial nephrectomy : effect of warm ischemia relative to quantity and quality of preserved kidney .
	manualset3
132493	6	406225	13	NULL	NULL	0	NULL	quality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal function after partial nephrectomy : effect of warm ischemia relative to quantity and quality of preserved kidney .
	manualset3
132494	7	406225	13	NULL	NULL	0	NULL	kidney	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal function after partial nephrectomy : effect of warm ischemia relative to quantity and quality of preserved kidney .
	manualset3
132495	1	406226	13	NULL	NULL	0	NULL	Renal impairment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal impairment is a frequent post-transplant complication that may occur for any number of reasons , including peri-operative ischemic events and nephrotoxicity secondary to anti-rejection medications .
	manualset3
132496	2	406226	13	NULL	NULL	0	NULL	post-transplant complication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal impairment is a frequent post-transplant complication that may occur for any number of reasons , including peri-operative ischemic events and nephrotoxicity secondary to anti-rejection medications .
	manualset3
132497	3	406226	13	NULL	NULL	0	NULL	number of reasons 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal impairment is a frequent post-transplant complication that may occur for any number of reasons , including peri-operative ischemic events and nephrotoxicity secondary to anti-rejection medications .
	manualset3
132498	4	406226	13	NULL	NULL	0	NULL	peri-operative ischemic events	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal impairment is a frequent post-transplant complication that may occur for any number of reasons , including peri-operative ischemic events and nephrotoxicity secondary to anti-rejection medications .
	manualset3
132499	5	406226	13	NULL	NULL	0	NULL	nephrotoxicity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal impairment is a frequent post-transplant complication that may occur for any number of reasons , including peri-operative ischemic events and nephrotoxicity secondary to anti-rejection medications .
	manualset3
132500	6	406226	13	NULL	NULL	NULL	NULL	anti-rejection medications	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Renal impairment is a frequent post-transplant complication that may occur for any number of reasons , including peri-operative ischemic events and nephrotoxicity secondary to anti-rejection medications .
	manualset3
132501	1	406227	13	NULL	NULL	0	NULL	Renal involvement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal involvement in the Laurence-Moon-Bardet-Biedl syndrome : report of five cases .
	manualset3
132502	2	406227	13	NULL	NULL	0	NULL	Laurence-Moon-Bardet-Biedl syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal involvement in the Laurence-Moon-Bardet-Biedl syndrome : report of five cases .
	manualset3
132503	3	406227	13	NULL	NULL	0	NULL	report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal involvement in the Laurence-Moon-Bardet-Biedl syndrome : report of five cases .
	manualset3
132504	4	406227	13	NULL	NULL	0	NULL	five cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal involvement in the Laurence-Moon-Bardet-Biedl syndrome : report of five cases .
	manualset3
132505	1	406228	13	NULL	NULL	0	NULL	Renal magnetic resonance angiography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal magnetic resonance angiography : an update .
	manualset3
134889	2	406228	13	NULL	NULL	0	NULL	update 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal magnetic resonance angiography : an update .
	manualset3
132506	1	406229	13	NULL	NULL	0	NULL	Renal transplantation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal transplantation is uncommon ( 700-800 per year ) , and it is likely that CAPD is of more value than in western countries as a dialysis technique .
	manualset3
132507	2	406229	13	NULL	NULL	0	NULL	700-800 per year 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal transplantation is uncommon ( 700-800 per year ) , and it is likely that CAPD is of more value than in western countries as a dialysis technique .
	manualset3
132508	3	406229	13	NULL	NULL	0	NULL	CAPD	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal transplantation is uncommon ( 700-800 per year ) , and it is likely that CAPD is of more value than in western countries as a dialysis technique .
	manualset3
132509	4	406229	13	NULL	NULL	0	NULL	value	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal transplantation is uncommon ( 700-800 per year ) , and it is likely that CAPD is of more value than in western countries as a dialysis technique .
	manualset3
132510	5	406229	13	NULL	NULL	0	NULL	western countries	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal transplantation is uncommon ( 700-800 per year ) , and it is likely that CAPD is of more value than in western countries as a dialysis technique .
	manualset3
132511	6	406229	13	NULL	NULL	0	NULL	dialysis technique	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal transplantation is uncommon ( 700-800 per year ) , and it is likely that CAPD is of more value than in western countries as a dialysis technique .
	manualset3
132512	1	406230	13	NULL	NULL	0	NULL	Renin release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Renin release and lipid peroxidation in renin granules of the rat .
	manualset3
132513	2	406230	13	NULL	NULL	0	NULL	lipid peroxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Renin release and lipid peroxidation in renin granules of the rat .
	manualset3
132514	3	406230	13	NULL	NULL	0	NULL	renin granules	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Renin release and lipid peroxidation in renin granules of the rat .
	manualset3
132515	4	406230	13	NULL	NULL	0	NULL	rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Renin release and lipid peroxidation in renin granules of the rat .
	manualset3
132516	1	406231	13	NULL	NULL	0	NULL	Reoperation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Reoperation for ascending aorta false aneurysm using deep hypothermia and circulatory arrest .
	manualset3
132517	2	406231	13	NULL	NULL	0	NULL	ascending aorta false aneurysm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reoperation for ascending aorta false aneurysm using deep hypothermia and circulatory arrest .
	manualset3
132518	3	406231	13	NULL	NULL	0	NULL	hypothermia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reoperation for ascending aorta false aneurysm using deep hypothermia and circulatory arrest .
	manualset3
132519	4	406231	13	NULL	NULL	0	NULL	circulatory arrest	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reoperation for ascending aorta false aneurysm using deep hypothermia and circulatory arrest .
	manualset3
132520	1	406232	13	NULL	NULL	0	NULL	Repair 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Repair of articular cartilage defect by autologous transplantation of basic fibroblast growth factor gene-transduced chondrocytes with adeno-associated virus vector .
	manualset3
132521	2	406232	13	NULL	NULL	0	NULL	articular cartilage defect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Repair of articular cartilage defect by autologous transplantation of basic fibroblast growth factor gene-transduced chondrocytes with adeno-associated virus vector .
	manualset3
132522	3	406232	13	NULL	NULL	0	NULL	autologous transplantation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Repair of articular cartilage defect by autologous transplantation of basic fibroblast growth factor gene-transduced chondrocytes with adeno-associated virus vector .
	manualset3
132523	4	406232	13	NULL	NULL	0	NULL	basic fibroblast growth factor gene-transduced chondrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Repair of articular cartilage defect by autologous transplantation of basic fibroblast growth factor gene-transduced chondrocytes with adeno-associated virus vector .
	manualset3
132524	5	406232	13	NULL	NULL	0	NULL	adeno-associated virus vector	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Repair of articular cartilage defect by autologous transplantation of basic fibroblast growth factor gene-transduced chondrocytes with adeno-associated virus vector .
	manualset3
132525	1	406233	13	NULL	NULL	0	NULL	Repair 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Repair was also examined in rat liver hepatocytes and non-parenchymal cells separately after administration of NDMA at non-AGT depleting doses .
	manualset3
132526	2	406233	13	NULL	NULL	0	NULL	rat liver hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Repair was also examined in rat liver hepatocytes and non-parenchymal cells separately after administration of NDMA at non-AGT depleting doses .
	manualset3
132527	3	406233	13	NULL	NULL	0	NULL	non-parenchymal cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Repair was also examined in rat liver hepatocytes and non-parenchymal cells separately after administration of NDMA at non-AGT depleting doses .
	manualset3
132528	4	406233	13	NULL	NULL	NULL	NULL	administration	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Repair was also examined in rat liver hepatocytes and non-parenchymal cells separately after administration of NDMA at non-AGT depleting doses .
	manualset3
132529	5	406233	13	NULL	NULL	0	NULL	NDMA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Repair was also examined in rat liver hepatocytes and non-parenchymal cells separately after administration of NDMA at non-AGT depleting doses .
	manualset3
132530	6	406233	13	NULL	NULL	0	NULL	non-AGT depleting doses	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Repair was also examined in rat liver hepatocytes and non-parenchymal cells separately after administration of NDMA at non-AGT depleting doses .
	manualset3
132531	1	406234	13	NULL	NULL	0	NULL	MR imaging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Repeat MR imaging done at six weeks showed complete resolution of the spinal SDH and partial resolution of the cranial SDH .
	manualset3
132532	2	406234	13	NULL	NULL	0	NULL	six weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Repeat MR imaging done at six weeks showed complete resolution of the spinal SDH and partial resolution of the cranial SDH .
	manualset3
132533	3	406234	13	NULL	NULL	0	NULL	resolution	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Repeat MR imaging done at six weeks showed complete resolution of the spinal SDH and partial resolution of the cranial SDH .
	manualset3
132534	4	406234	13	NULL	NULL	0	NULL	spinal SDH 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Repeat MR imaging done at six weeks showed complete resolution of the spinal SDH and partial resolution of the cranial SDH .
	manualset3
132535	5	406234	13	NULL	NULL	0	NULL	resolution	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Repeat MR imaging done at six weeks showed complete resolution of the spinal SDH and partial resolution of the cranial SDH .
	manualset3
132536	6	406234	13	NULL	NULL	0	NULL	cranial SDH	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Repeat MR imaging done at six weeks showed complete resolution of the spinal SDH and partial resolution of the cranial SDH .
	manualset3
132537	1	406235	13	NULL	NULL	0	NULL	surgical resection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Repeated surgical resection and stereotactic radiosurgery was performed , but she died 44 months after the initial nephroureterectomy due to the relapse of brain metastasis .
	manualset3
132538	2	406235	13	NULL	NULL	0	NULL	stereotactic radiosurgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Repeated surgical resection and stereotactic radiosurgery was performed , but she died 44 months after the initial nephroureterectomy due to the relapse of brain metastasis .
	manualset3
132539	3	406235	13	NULL	NULL	0	NULL	44 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Repeated surgical resection and stereotactic radiosurgery was performed , but she died 44 months after the initial nephroureterectomy due to the relapse of brain metastasis .
	manualset3
132540	4	406235	13	NULL	NULL	0	NULL	nephroureterectomy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Repeated surgical resection and stereotactic radiosurgery was performed , but she died 44 months after the initial nephroureterectomy due to the relapse of brain metastasis .
	manualset3
132541	5	406235	13	NULL	NULL	0	NULL	relapse of brain metastasis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Repeated surgical resection and stereotactic radiosurgery was performed , but she died 44 months after the initial nephroureterectomy due to the relapse of brain metastasis .
	manualset3
132542	1	406236	13	NULL	NULL	0	NULL	test 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Repeating the test using a different D-dimer assay as well as the measurement of other fibrinolysis markers confirmed the diagnosis of DIC .
	manualset3
132543	2	406236	13	NULL	NULL	0	NULL	D-dimer assay 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Repeating the test using a different D-dimer assay as well as the measurement of other fibrinolysis markers confirmed the diagnosis of DIC .
	manualset3
132544	3	406236	13	NULL	NULL	0	NULL	measurement	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Repeating the test using a different D-dimer assay as well as the measurement of other fibrinolysis markers confirmed the diagnosis of DIC .
	manualset3
132545	4	406236	13	NULL	NULL	0	NULL	fibrinolysis markers	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Repeating the test using a different D-dimer assay as well as the measurement of other fibrinolysis markers confirmed the diagnosis of DIC .
	manualset3
132546	5	406236	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Repeating the test using a different D-dimer assay as well as the measurement of other fibrinolysis markers confirmed the diagnosis of DIC .
	manualset3
132547	6	406236	13	NULL	NULL	0	NULL	DIC 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Repeating the test using a different D-dimer assay as well as the measurement of other fibrinolysis markers confirmed the diagnosis of DIC .
	manualset3
132548	1	406237	13	NULL	NULL	0	NULL	multi-centered cooperative study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A multi-centered cooperative study is being undertaken to determine the role of carotid endarterectomy in the treatment of asymptomatic carotid stenosis .
	manualset3
132549	2	406237	13	NULL	NULL	0	NULL	role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A multi-centered cooperative study is being undertaken to determine the role of carotid endarterectomy in the treatment of asymptomatic carotid stenosis .
	manualset3
132550	3	406237	13	NULL	NULL	0	NULL	carotid endarterectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A multi-centered cooperative study is being undertaken to determine the role of carotid endarterectomy in the treatment of asymptomatic carotid stenosis .
	manualset3
132551	4	406237	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A multi-centered cooperative study is being undertaken to determine the role of carotid endarterectomy in the treatment of asymptomatic carotid stenosis .
	manualset3
132552	5	406237	13	NULL	NULL	0	NULL	asymptomatic carotid stenosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A multi-centered cooperative study is being undertaken to determine the role of carotid endarterectomy in the treatment of asymptomatic carotid stenosis .
	manualset3
132553	1	406238	13	NULL	NULL	0	NULL	Repetition rate evolution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Repetition rate evolution and timing jitter increase is attributed to the coupling between the dominant and the secondary supermodes .
	manualset3
132554	2	406238	13	NULL	NULL	0	NULL	timing jitter increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Repetition rate evolution and timing jitter increase is attributed to the coupling between the dominant and the secondary supermodes .
	manualset3
132555	3	406238	13	NULL	NULL	0	NULL	coupling 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Repetition rate evolution and timing jitter increase is attributed to the coupling between the dominant and the secondary supermodes .
	manualset3
132556	4	406238	13	NULL	NULL	0	NULL	dominant supermodes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Repetition rate evolution and timing jitter increase is attributed to the coupling between the dominant and the secondary supermodes .
	manualset3
132557	5	406238	13	NULL	NULL	0	NULL	secondary supermodes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Repetition rate evolution and timing jitter increase is attributed to the coupling between the dominant and the secondary supermodes .
	manualset3
132558	1	406239	13	NULL	NULL	0	NULL	Repetitive operation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Repetitive operation of switchless transverse flow transversely excited atmosphere CO2 lasers .
	manualset3
132559	2	406239	13	NULL	NULL	0	NULL	switchless transverse flow	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Repetitive operation of switchless transverse flow transversely excited atmosphere CO2 lasers .
	manualset3
132560	3	406239	13	NULL	NULL	0	NULL	atmosphere	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Repetitive operation of switchless transverse flow transversely excited atmosphere CO2 lasers .
	manualset3
132561	4	406239	13	NULL	NULL	0	NULL	CO2 lasers	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Repetitive operation of switchless transverse flow transversely excited atmosphere CO2 lasers .
	manualset3
132562	1	406240	13	NULL	NULL	0	NULL	Repetitive stimulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Repetitive stimulation ( greater than 5Hz ) led to summation of EJPs , which evoked spikes and vasoconstriction .
	manualset3
132563	2	406240	13	NULL	NULL	0	NULL	5Hz	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Repetitive stimulation ( greater than 5Hz ) led to summation of EJPs , which evoked spikes and vasoconstriction .
	manualset3
132564	3	406240	13	NULL	NULL	0	NULL	summation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Repetitive stimulation ( greater than 5Hz ) led to summation of EJPs , which evoked spikes and vasoconstriction .
	manualset3
132565	4	406240	13	NULL	NULL	0	NULL	EJPs	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Repetitive stimulation ( greater than 5Hz ) led to summation of EJPs , which evoked spikes and vasoconstriction .
	manualset3
132566	5	406240	13	NULL	NULL	0	NULL	spikes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Repetitive stimulation ( greater than 5Hz ) led to summation of EJPs , which evoked spikes and vasoconstriction .
	manualset3
132567	6	406240	13	NULL	NULL	0	NULL	vasoconstriction 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Repetitive stimulation ( greater than 5Hz ) led to summation of EJPs , which evoked spikes and vasoconstriction .
	manualset3
132568	1	406241	13	NULL	NULL	0	NULL	Repetitive strain disorder	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Repetitive strain disorder : towards diagnostic criteria .
	manualset3
132569	2	406241	13	NULL	NULL	0	NULL	diagnostic criteria	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Repetitive strain disorder : towards diagnostic criteria .
	manualset3
132570	1	406242	13	NULL	NULL	0	NULL	Replacement	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Replacement of the damaged chondral surface of the patella is often difficult because of the high mechanical stresses and the relatively thin cancellous surfaces .
	manualset3
132571	2	406242	13	NULL	NULL	0	NULL	chondral surface	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Replacement of the damaged chondral surface of the patella is often difficult because of the high mechanical stresses and the relatively thin cancellous surfaces .
	manualset3
132572	3	406242	13	NULL	NULL	0	NULL	patella	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Replacement of the damaged chondral surface of the patella is often difficult because of the high mechanical stresses and the relatively thin cancellous surfaces .
	manualset3
132573	4	406242	13	NULL	NULL	0	NULL	mechanical stresses	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Replacement of the damaged chondral surface of the patella is often difficult because of the high mechanical stresses and the relatively thin cancellous surfaces .
	manualset3
132574	5	406242	13	NULL	NULL	0	NULL	cancellous surfaces 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Replacement of the damaged chondral surface of the patella is often difficult because of the high mechanical stresses and the relatively thin cancellous surfaces .
	manualset3
132575	1	406243	13	NULL	NULL	0	NULL	Replication kinetics	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Replication kinetics of Salmonella enteritidis in internal organs of ducklings after oral challenge : a quantitative time-course study using real-time PCR .
	manualset3
132576	2	406243	13	NULL	NULL	0	NULL	Salmonella enteritidis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Replication kinetics of Salmonella enteritidis in internal organs of ducklings after oral challenge : a quantitative time-course study using real-time PCR .
	manualset3
132577	3	406243	13	NULL	NULL	0	NULL	internal organs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Replication kinetics of Salmonella enteritidis in internal organs of ducklings after oral challenge : a quantitative time-course study using real-time PCR .
	manualset3
132578	4	406243	13	NULL	NULL	0	NULL	ducklings 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Replication kinetics of Salmonella enteritidis in internal organs of ducklings after oral challenge : a quantitative time-course study using real-time PCR .
	manualset3
132579	5	406243	13	NULL	NULL	0	NULL	oral challenge	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Replication kinetics of Salmonella enteritidis in internal organs of ducklings after oral challenge : a quantitative time-course study using real-time PCR .
	manualset3
132580	6	406243	13	NULL	NULL	0	NULL	quantitative time-course study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Replication kinetics of Salmonella enteritidis in internal organs of ducklings after oral challenge : a quantitative time-course study using real-time PCR .
	manualset3
132581	7	406243	13	NULL	NULL	0	NULL	real-time PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Replication kinetics of Salmonella enteritidis in internal organs of ducklings after oral challenge : a quantitative time-course study using real-time PCR .
	manualset3
132582	1	406244	13	NULL	NULL	0	NULL	Replication	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Replication of circular N15-based miniplasmids requires the only gene repA that encodes multidomain protein homologous to replication proteins of bacterial plasmids replicated by theta-mechanism , particularly , phage P4 alpha-replication protein .
	manualset3
132583	2	406244	13	NULL	NULL	0	NULL	circular N15-based miniplasmids 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Replication of circular N15-based miniplasmids requires the only gene repA that encodes multidomain protein homologous to replication proteins of bacterial plasmids replicated by theta-mechanism , particularly , phage P4 alpha-replication protein .
	manualset3
132584	3	406244	13	NULL	NULL	0	NULL	gene repA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Replication of circular N15-based miniplasmids requires the only gene repA that encodes multidomain protein homologous to replication proteins of bacterial plasmids replicated by theta-mechanism , particularly , phage P4 alpha-replication protein .
	manualset3
132585	4	406244	13	NULL	NULL	0	NULL	multidomain protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Replication of circular N15-based miniplasmids requires the only gene repA that encodes multidomain protein homologous to replication proteins of bacterial plasmids replicated by theta-mechanism , particularly , phage P4 alpha-replication protein .
	manualset3
132586	5	406244	13	NULL	NULL	0	NULL	replication proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Replication of circular N15-based miniplasmids requires the only gene repA that encodes multidomain protein homologous to replication proteins of bacterial plasmids replicated by theta-mechanism , particularly , phage P4 alpha-replication protein .
	manualset3
132587	6	406244	13	NULL	NULL	0	NULL	bacterial plasmids 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Replication of circular N15-based miniplasmids requires the only gene repA that encodes multidomain protein homologous to replication proteins of bacterial plasmids replicated by theta-mechanism , particularly , phage P4 alpha-replication protein .
	manualset3
132588	7	406244	13	NULL	NULL	0	NULL	theta-mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Replication of circular N15-based miniplasmids requires the only gene repA that encodes multidomain protein homologous to replication proteins of bacterial plasmids replicated by theta-mechanism , particularly , phage P4 alpha-replication protein .
	manualset3
132589	8	406244	13	NULL	NULL	0	NULL	phage P4 alpha-replication protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Replication of circular N15-based miniplasmids requires the only gene repA that encodes multidomain protein homologous to replication proteins of bacterial plasmids replicated by theta-mechanism , particularly , phage P4 alpha-replication protein .
	manualset3
132665	1	406245	13	NULL	NULL	0	NULL	Replication 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Replication of damaged DNA is essential in all organisms and is potentially achieved by several mechanisms .
	manualset3
132666	2	406245	13	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Replication of damaged DNA is essential in all organisms and is potentially achieved by several mechanisms .
	manualset3
132667	3	406245	13	NULL	NULL	0	NULL	organisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Replication of damaged DNA is essential in all organisms and is potentially achieved by several mechanisms .
	manualset3
132668	4	406245	13	NULL	NULL	0	NULL	mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Replication of damaged DNA is essential in all organisms and is potentially achieved by several mechanisms .
	manualset3
132669	1	406246	13	NULL	NULL	0	NULL	Replication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Replication of the most significantly associated polymorphisms in multiple populations with distinctive genetic backgrounds and lifestyles is crucial to the understanding of the pathophysiology of a multifactorial disease like CAD .
	manualset3
132674	2	406246	13	NULL	NULL	0	NULL	polymorphisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Replication of the most significantly associated polymorphisms in multiple populations with distinctive genetic backgrounds and lifestyles is crucial to the understanding of the pathophysiology of a multifactorial disease like CAD .
	manualset3
132675	3	406246	13	NULL	NULL	0	NULL	multiple populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Replication of the most significantly associated polymorphisms in multiple populations with distinctive genetic backgrounds and lifestyles is crucial to the understanding of the pathophysiology of a multifactorial disease like CAD .
	manualset3
132676	4	406246	13	NULL	NULL	0	NULL	genetic backgrounds 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Replication of the most significantly associated polymorphisms in multiple populations with distinctive genetic backgrounds and lifestyles is crucial to the understanding of the pathophysiology of a multifactorial disease like CAD .
	manualset3
132677	5	406246	13	NULL	NULL	0	NULL	lifestyles 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Replication of the most significantly associated polymorphisms in multiple populations with distinctive genetic backgrounds and lifestyles is crucial to the understanding of the pathophysiology of a multifactorial disease like CAD .
	manualset3
132678	6	406246	13	NULL	NULL	0	NULL	understanding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Replication of the most significantly associated polymorphisms in multiple populations with distinctive genetic backgrounds and lifestyles is crucial to the understanding of the pathophysiology of a multifactorial disease like CAD .
	manualset3
132679	7	406246	13	NULL	NULL	0	NULL	pathophysiology 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Replication of the most significantly associated polymorphisms in multiple populations with distinctive genetic backgrounds and lifestyles is crucial to the understanding of the pathophysiology of a multifactorial disease like CAD .
	manualset3
132680	8	406246	13	NULL	NULL	0	NULL	multifactorial disease like CAD 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Replication of the most significantly associated polymorphisms in multiple populations with distinctive genetic backgrounds and lifestyles is crucial to the understanding of the pathophysiology of a multifactorial disease like CAD .
	manualset3
132681	1	406247	13	NULL	NULL	0	NULL	multicenter study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A multicenter study on the effects of lanthanum carbonate ( Fosrenol ) and calcium carbonate on renal bone disease in dialysis patients .
	manualset3
132682	2	406247	13	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A multicenter study on the effects of lanthanum carbonate ( Fosrenol ) and calcium carbonate on renal bone disease in dialysis patients .
	manualset3
132683	3	406247	13	NULL	NULL	0	NULL	 lanthanum carbonate ( Fosrenol )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A multicenter study on the effects of lanthanum carbonate ( Fosrenol ) and calcium carbonate on renal bone disease in dialysis patients .
	manualset3
132684	4	406247	13	NULL	NULL	0	NULL	calcium carbonate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A multicenter study on the effects of lanthanum carbonate ( Fosrenol ) and calcium carbonate on renal bone disease in dialysis patients .
	manualset3
132685	5	406247	13	NULL	NULL	0	NULL	renal bone disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A multicenter study on the effects of lanthanum carbonate ( Fosrenol ) and calcium carbonate on renal bone disease in dialysis patients .
	manualset3
132686	6	406247	13	NULL	NULL	0	NULL	dialysis patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A multicenter study on the effects of lanthanum carbonate ( Fosrenol ) and calcium carbonate on renal bone disease in dialysis patients .
	manualset3
132687	1	406248	13	NULL	NULL	0	NULL	Replicative fitness	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Replicative fitness of CCR5-using and CXCR4-using human immunodeficiency virus type 1 biological clones .
	manualset3
132688	2	406248	13	NULL	NULL	0	NULL	 CCR5-using human immunodeficiency virus type 1 biological clones	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Replicative fitness of CCR5-using and CXCR4-using human immunodeficiency virus type 1 biological clones .
	manualset3
132689	3	406248	13	NULL	NULL	0	NULL	CXCR4-using human immunodeficiency virus type 1 biological clones	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Replicative fitness of CCR5-using and CXCR4-using human immunodeficiency virus type 1 biological clones .
	manualset3
132690	1	406249	13	NULL	NULL	0	NULL	Reported data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Reported data indicated that such a panel of investigations is useful to better define the non-specific immunological phenomenons which take place in this active pathological tissue .
	manualset3
132691	2	406249	13	NULL	NULL	0	NULL	panel of investigations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Reported data indicated that such a panel of investigations is useful to better define the non-specific immunological phenomenons which take place in this active pathological tissue .
	manualset3
132692	3	406249	13	NULL	NULL	0	NULL	non-specific immunological phenomenons	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reported data indicated that such a panel of investigations is useful to better define the non-specific immunological phenomenons which take place in this active pathological tissue .
	manualset3
132693	4	406249	13	NULL	NULL	0	NULL	active pathological tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Reported data indicated that such a panel of investigations is useful to better define the non-specific immunological phenomenons which take place in this active pathological tissue .
	manualset3
132694	1	406250	13	NULL	NULL	0	NULL	Reporter gene assays 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Reporter gene assays showed HSV-induced RANTES production to be regulated at the transcriptional level .
	manualset3
132695	2	406250	13	NULL	NULL	0	NULL	HSV-induced RANTES production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reporter gene assays showed HSV-induced RANTES production to be regulated at the transcriptional level .
	manualset3
132696	3	406250	13	NULL	NULL	0	NULL	transcriptional level	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reporter gene assays showed HSV-induced RANTES production to be regulated at the transcriptional level .
	manualset3
132697	1	406251	13	NULL	NULL	0	NULL	Reports 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports from Asia of decreased Salmonella typhi resistance to chloramphenicol , attributed to restricted antibiotic usage , may indicate a reversal of the usual trend .
	manualset3
132698	2	406251	13	NULL	NULL	0	NULL	Asia	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports from Asia of decreased Salmonella typhi resistance to chloramphenicol , attributed to restricted antibiotic usage , may indicate a reversal of the usual trend .
	manualset3
132699	3	406251	13	NULL	NULL	0	NULL	Salmonella typhi resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports from Asia of decreased Salmonella typhi resistance to chloramphenicol , attributed to restricted antibiotic usage , may indicate a reversal of the usual trend .
	manualset3
132700	4	406251	13	NULL	NULL	0	NULL	chloramphenicol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports from Asia of decreased Salmonella typhi resistance to chloramphenicol , attributed to restricted antibiotic usage , may indicate a reversal of the usual trend .
	manualset3
132701	5	406251	13	NULL	NULL	0	NULL	antibiotic usage	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports from Asia of decreased Salmonella typhi resistance to chloramphenicol , attributed to restricted antibiotic usage , may indicate a reversal of the usual trend .
	manualset3
132702	6	406251	13	NULL	NULL	0	NULL	reversal 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports from Asia of decreased Salmonella typhi resistance to chloramphenicol , attributed to restricted antibiotic usage , may indicate a reversal of the usual trend .
	manualset3
132703	7	406251	13	NULL	NULL	0	NULL	trend	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports from Asia of decreased Salmonella typhi resistance to chloramphenicol , attributed to restricted antibiotic usage , may indicate a reversal of the usual trend .
	manualset3
132704	1	406252	13	NULL	NULL	0	NULL	Reports	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports of RNAi screens for the identification of novel genes implicated in apoptosis , cell division , and drug resistance support the enormous promise of this technology .
	manualset3
132705	2	406252	13	NULL	NULL	0	NULL	RNAi screens	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports of RNAi screens for the identification of novel genes implicated in apoptosis , cell division , and drug resistance support the enormous promise of this technology .
	manualset3
132706	3	406252	13	NULL	NULL	0	NULL	identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports of RNAi screens for the identification of novel genes implicated in apoptosis , cell division , and drug resistance support the enormous promise of this technology .
	manualset3
132707	4	406252	13	NULL	NULL	0	NULL	novel genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports of RNAi screens for the identification of novel genes implicated in apoptosis , cell division , and drug resistance support the enormous promise of this technology .
	manualset3
132708	5	406252	13	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports of RNAi screens for the identification of novel genes implicated in apoptosis , cell division , and drug resistance support the enormous promise of this technology .
	manualset3
132709	6	406252	13	NULL	NULL	0	NULL	cell division	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports of RNAi screens for the identification of novel genes implicated in apoptosis , cell division , and drug resistance support the enormous promise of this technology .
	manualset3
132710	7	406252	13	NULL	NULL	0	NULL	drug resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports of RNAi screens for the identification of novel genes implicated in apoptosis , cell division , and drug resistance support the enormous promise of this technology .
	manualset3
132712	9	406252	13	NULL	NULL	0	NULL	promise 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports of RNAi screens for the identification of novel genes implicated in apoptosis , cell division , and drug resistance support the enormous promise of this technology .
	manualset3
132713	10	406252	13	NULL	NULL	0	NULL	technology 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports of RNAi screens for the identification of novel genes implicated in apoptosis , cell division , and drug resistance support the enormous promise of this technology .
	manualset3
132714	1	406253	13	NULL	NULL	0	NULL	Reports 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports of leukemia and brain cancer among men in electrical occupations suggest a small increase in risk , but most previous studies have failed to classify magnetic field exposure accurately or to consider potential confounders .
	manualset3
132715	2	406253	13	NULL	NULL	0	NULL	leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports of leukemia and brain cancer among men in electrical occupations suggest a small increase in risk , but most previous studies have failed to classify magnetic field exposure accurately or to consider potential confounders .
	manualset3
132716	3	406253	13	NULL	NULL	0	NULL	brain cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports of leukemia and brain cancer among men in electrical occupations suggest a small increase in risk , but most previous studies have failed to classify magnetic field exposure accurately or to consider potential confounders .
	manualset3
132717	4	406253	13	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports of leukemia and brain cancer among men in electrical occupations suggest a small increase in risk , but most previous studies have failed to classify magnetic field exposure accurately or to consider potential confounders .
	manualset3
132718	5	406253	13	NULL	NULL	0	NULL	electrical occupations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports of leukemia and brain cancer among men in electrical occupations suggest a small increase in risk , but most previous studies have failed to classify magnetic field exposure accurately or to consider potential confounders .
	manualset3
132719	6	406253	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports of leukemia and brain cancer among men in electrical occupations suggest a small increase in risk , but most previous studies have failed to classify magnetic field exposure accurately or to consider potential confounders .
	manualset3
132720	7	406253	13	NULL	NULL	0	NULL	risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports of leukemia and brain cancer among men in electrical occupations suggest a small increase in risk , but most previous studies have failed to classify magnetic field exposure accurately or to consider potential confounders .
	manualset3
132721	8	406253	13	NULL	NULL	0	NULL	previous studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports of leukemia and brain cancer among men in electrical occupations suggest a small increase in risk , but most previous studies have failed to classify magnetic field exposure accurately or to consider potential confounders .
	manualset3
132722	9	406253	13	NULL	NULL	0	NULL	magnetic field exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports of leukemia and brain cancer among men in electrical occupations suggest a small increase in risk , but most previous studies have failed to classify magnetic field exposure accurately or to consider potential confounders .
	manualset3
132723	10	406253	13	NULL	NULL	0	NULL	confounders	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports of leukemia and brain cancer among men in electrical occupations suggest a small increase in risk , but most previous studies have failed to classify magnetic field exposure accurately or to consider potential confounders .
	manualset3
132724	1	406254	13	NULL	NULL	0	NULL	Representation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Representation and legitimacy in health policy formulation at a national level : perspectives from a study of health technology eligibility procedures in the United Kingdom .
	manualset3
132725	2	406254	13	NULL	NULL	0	NULL	legitimacy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Representation and legitimacy in health policy formulation at a national level : perspectives from a study of health technology eligibility procedures in the United Kingdom .
	manualset3
132726	3	406254	13	NULL	NULL	0	NULL	health policy formulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Representation and legitimacy in health policy formulation at a national level : perspectives from a study of health technology eligibility procedures in the United Kingdom .
	manualset3
132727	4	406254	13	NULL	NULL	0	NULL	national level	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Representation and legitimacy in health policy formulation at a national level : perspectives from a study of health technology eligibility procedures in the United Kingdom .
	manualset3
132728	5	406254	13	NULL	NULL	NULL	NULL	perspectives	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Representation and legitimacy in health policy formulation at a national level : perspectives from a study of health technology eligibility procedures in the United Kingdom .
	manualset3
132729	6	406254	13	NULL	NULL	0	NULL	study 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Representation and legitimacy in health policy formulation at a national level : perspectives from a study of health technology eligibility procedures in the United Kingdom .
	manualset3
132730	7	406254	13	NULL	NULL	0	NULL	health technology eligibility procedures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Representation and legitimacy in health policy formulation at a national level : perspectives from a study of health technology eligibility procedures in the United Kingdom .
	manualset3
132731	8	406254	13	NULL	NULL	0	NULL	United Kingdom	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Representation and legitimacy in health policy formulation at a national level : perspectives from a study of health technology eligibility procedures in the United Kingdom .
	manualset3
132732	1	406255	13	NULL	NULL	0	NULL	Representative data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Representative data are presented from studies of DNA conformation and architecture in polytene chromosomes and from studies of receptor-mediated endocytosis , calcium distribution , and the organization of the contractile apparatus in muscle cells .
	manualset3
132733	2	406255	13	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Representative data are presented from studies of DNA conformation and architecture in polytene chromosomes and from studies of receptor-mediated endocytosis , calcium distribution , and the organization of the contractile apparatus in muscle cells .
	manualset3
132734	3	406255	13	NULL	NULL	0	NULL	DNA conformation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Representative data are presented from studies of DNA conformation and architecture in polytene chromosomes and from studies of receptor-mediated endocytosis , calcium distribution , and the organization of the contractile apparatus in muscle cells .
	manualset3
132735	4	406255	13	NULL	NULL	0	NULL	architecture	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Representative data are presented from studies of DNA conformation and architecture in polytene chromosomes and from studies of receptor-mediated endocytosis , calcium distribution , and the organization of the contractile apparatus in muscle cells .
	manualset3
132736	5	406255	13	NULL	NULL	0	NULL	polytene chromosomes	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Representative data are presented from studies of DNA conformation and architecture in polytene chromosomes and from studies of receptor-mediated endocytosis , calcium distribution , and the organization of the contractile apparatus in muscle cells .
	manualset3
132737	6	406255	13	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Representative data are presented from studies of DNA conformation and architecture in polytene chromosomes and from studies of receptor-mediated endocytosis , calcium distribution , and the organization of the contractile apparatus in muscle cells .
	manualset3
132738	7	406255	13	NULL	NULL	0	NULL	receptor-mediated endocytosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Representative data are presented from studies of DNA conformation and architecture in polytene chromosomes and from studies of receptor-mediated endocytosis , calcium distribution , and the organization of the contractile apparatus in muscle cells .
	manualset3
132739	8	406255	13	NULL	NULL	0	NULL	calcium distribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Representative data are presented from studies of DNA conformation and architecture in polytene chromosomes and from studies of receptor-mediated endocytosis , calcium distribution , and the organization of the contractile apparatus in muscle cells .
	manualset3
132740	9	406255	13	NULL	NULL	0	NULL	organization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Representative data are presented from studies of DNA conformation and architecture in polytene chromosomes and from studies of receptor-mediated endocytosis , calcium distribution , and the organization of the contractile apparatus in muscle cells .
	manualset3
132741	10	406255	13	NULL	NULL	0	NULL	contractile apparatus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Representative data are presented from studies of DNA conformation and architecture in polytene chromosomes and from studies of receptor-mediated endocytosis , calcium distribution , and the organization of the contractile apparatus in muscle cells .
	manualset3
132742	11	406255	13	NULL	NULL	0	NULL	muscle cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Representative data are presented from studies of DNA conformation and architecture in polytene chromosomes and from studies of receptor-mediated endocytosis , calcium distribution , and the organization of the contractile apparatus in muscle cells .
	manualset3
132743	1	406256	13	NULL	NULL	0	NULL	Representativity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Representativity of a mid-lake surface water chemistry sample .
	manualset3
132744	2	406256	13	NULL	NULL	0	NULL	mid-lake surface water chemistry sample	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Representativity of a mid-lake surface water chemistry sample .
	manualset3
132745	1	406257	13	NULL	NULL	0	NULL	 multicultural study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A multicultural study of stereotyping in English-speaking countries .
	manualset3
132746	2	406257	13	NULL	NULL	0	NULL	English-speaking countries 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A multicultural study of stereotyping in English-speaking countries .
	manualset3
134890	3	406257	13	NULL	NULL	0	NULL	stereotyping	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A multicultural study of stereotyping in English-speaking countries .
	manualset3
132747	1	406258	13	NULL	NULL	0	NULL	Research 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Research addressing digestible Lys requirement data of modern broilers from 4 to 6 wk of age is limited .
	manualset3
132748	2	406258	13	NULL	NULL	NULL	NULL	Lys requirement data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Research addressing digestible Lys requirement data of modern broilers from 4 to 6 wk of age is limited .
	manualset3
132749	3	406258	13	NULL	NULL	0	NULL	modern broilers	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Research addressing digestible Lys requirement data of modern broilers from 4 to 6 wk of age is limited .
	manualset3
132750	4	406258	13	NULL	NULL	0	NULL	4 to 6 wk of age	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Research addressing digestible Lys requirement data of modern broilers from 4 to 6 wk of age is limited .
	manualset3
132751	1	406259	13	NULL	NULL	0	NULL	Research issues 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Research issues related to oral health expenditures and financing oral health care for the aging veteran .
	manualset3
132752	2	406259	13	NULL	NULL	0	NULL	oral health expenditures	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Research issues related to oral health expenditures and financing oral health care for the aging veteran .
	manualset3
132754	4	406259	13	NULL	NULL	0	NULL	oral health care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Research issues related to oral health expenditures and financing oral health care for the aging veteran .
	manualset3
132755	5	406259	13	NULL	NULL	0	NULL	veteran	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Research issues related to oral health expenditures and financing oral health care for the aging veteran .
	manualset3
132756	1	406260	13	NULL	NULL	0	NULL	Research proposals	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Research proposals and debates : a teaching strategy .
	manualset3
132757	2	406260	13	NULL	NULL	0	NULL	debates	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Research proposals and debates : a teaching strategy .
	manualset3
132758	3	406260	13	NULL	NULL	0	NULL	teaching strategy	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Research proposals and debates : a teaching strategy .
	manualset3
132759	1	406261	13	NULL	NULL	0	NULL	Research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Research suggests a link between antipsychotics , ECG abnormalities ( QT prolongation ) and increased sudden cardiac mortality rates .
	manualset3
132760	2	406261	13	NULL	NULL	0	NULL	link 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Research suggests a link between antipsychotics , ECG abnormalities ( QT prolongation ) and increased sudden cardiac mortality rates .
	manualset3
132761	3	406261	13	NULL	NULL	0	NULL	antipsychotics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Research suggests a link between antipsychotics , ECG abnormalities ( QT prolongation ) and increased sudden cardiac mortality rates .
	manualset3
132762	4	406261	13	NULL	NULL	0	NULL	ECG abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Research suggests a link between antipsychotics , ECG abnormalities ( QT prolongation ) and increased sudden cardiac mortality rates .
	manualset3
132763	5	406261	13	NULL	NULL	0	NULL	QT prolongation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Research suggests a link between antipsychotics , ECG abnormalities ( QT prolongation ) and increased sudden cardiac mortality rates .
	manualset3
132764	6	406261	13	NULL	NULL	0	NULL	cardiac mortality rates	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Research suggests a link between antipsychotics , ECG abnormalities ( QT prolongation ) and increased sudden cardiac mortality rates .
	manualset3
132770	1	406262	13	NULL	NULL	0	NULL	Research 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Research suggests paranoia among persons with schizophrenia may be the result of a number of different psychological processes including deficits in theory of mind ( ToM ) and social anxiety .
	manualset3
132771	2	406262	13	NULL	NULL	0	NULL	paranoia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Research suggests paranoia among persons with schizophrenia may be the result of a number of different psychological processes including deficits in theory of mind ( ToM ) and social anxiety .
	manualset3
132772	3	406262	13	NULL	NULL	0	NULL	persons	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Research suggests paranoia among persons with schizophrenia may be the result of a number of different psychological processes including deficits in theory of mind ( ToM ) and social anxiety .
	manualset3
132773	4	406262	13	NULL	NULL	0	NULL	schizophrenia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Research suggests paranoia among persons with schizophrenia may be the result of a number of different psychological processes including deficits in theory of mind ( ToM ) and social anxiety .
	manualset3
132775	5	406262	13	NULL	NULL	0	NULL	result 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Research suggests paranoia among persons with schizophrenia may be the result of a number of different psychological processes including deficits in theory of mind ( ToM ) and social anxiety .
	manualset3
132776	6	406262	13	NULL	NULL	0	NULL	number	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Research suggests paranoia among persons with schizophrenia may be the result of a number of different psychological processes including deficits in theory of mind ( ToM ) and social anxiety .
	manualset3
132777	7	406262	13	NULL	NULL	0	NULL	psychological processes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Research suggests paranoia among persons with schizophrenia may be the result of a number of different psychological processes including deficits in theory of mind ( ToM ) and social anxiety .
	manualset3
132778	8	406262	13	NULL	NULL	0	NULL	deficits 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Research suggests paranoia among persons with schizophrenia may be the result of a number of different psychological processes including deficits in theory of mind ( ToM ) and social anxiety .
	manualset3
132779	9	406262	13	NULL	NULL	NULL	NULL	theory of mind ( ToM ) 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Research suggests paranoia among persons with schizophrenia may be the result of a number of different psychological processes including deficits in theory of mind ( ToM ) and social anxiety .
	manualset3
132780	10	406262	13	NULL	NULL	0	NULL	social anxiety 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Research suggests paranoia among persons with schizophrenia may be the result of a number of different psychological processes including deficits in theory of mind ( ToM ) and social anxiety .
	manualset3
132781	1	406263	13	NULL	NULL	0	NULL	multidisciplinary team approach	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A multidisciplinary team approach including provocative angiography and an endovascular stent saved the life of the patient .
	manualset3
132782	2	406263	13	NULL	NULL	0	NULL	provocative angiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A multidisciplinary team approach including provocative angiography and an endovascular stent saved the life of the patient .
	manualset3
132783	3	406263	13	NULL	NULL	0	NULL	endovascular stent	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A multidisciplinary team approach including provocative angiography and an endovascular stent saved the life of the patient .
	manualset3
132784	4	406263	13	NULL	NULL	0	NULL	life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A multidisciplinary team approach including provocative angiography and an endovascular stent saved the life of the patient .
	manualset3
132785	5	406263	13	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A multidisciplinary team approach including provocative angiography and an endovascular stent saved the life of the patient .
	manualset3
132786	1	406264	13	NULL	NULL	0	NULL	Research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Research over the last several decades has revealed that satellite divergence can serve as a formidable reproductive barrier between sibling species .
	manualset3
132787	2	406264	13	NULL	NULL	0	NULL	several decades	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Research over the last several decades has revealed that satellite divergence can serve as a formidable reproductive barrier between sibling species .
	manualset3
132788	3	406264	13	NULL	NULL	NULL	NULL	satellite divergence	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Research over the last several decades has revealed that satellite divergence can serve as a formidable reproductive barrier between sibling species .
	manualset3
132789	4	406264	13	NULL	NULL	NULL	NULL	reproductive barrier	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Research over the last several decades has revealed that satellite divergence can serve as a formidable reproductive barrier between sibling species .
	manualset3
132790	5	406264	13	NULL	NULL	0	NULL	sibling species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Research over the last several decades has revealed that satellite divergence can serve as a formidable reproductive barrier between sibling species .
	manualset3
132791	1	406265	13	NULL	NULL	0	NULL	Research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Research in mental retardation : toward an etiologic approach .
	manualset3
132792	2	406265	13	NULL	NULL	0	NULL	mental retardation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Research in mental retardation : toward an etiologic approach .
	manualset3
132793	3	406265	13	NULL	NULL	0	NULL	etiologic approach	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Research in mental retardation : toward an etiologic approach .
	manualset3
132794	1	406266	13	NULL	NULL	0	NULL	Researchers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Researchers are now taking 2P microscopy beyond the study of model antigen systems ( e.g. ovalbumin immunization ) and are applying the technique to examine infection in vivo .
	manualset3
132795	2	406266	13	NULL	NULL	0	NULL	 2P microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Researchers are now taking 2P microscopy beyond the study of model antigen systems ( e.g. ovalbumin immunization ) and are applying the technique to examine infection in vivo .
	manualset3
132796	3	406266	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Researchers are now taking 2P microscopy beyond the study of model antigen systems ( e.g. ovalbumin immunization ) and are applying the technique to examine infection in vivo .
	manualset3
132797	4	406266	13	NULL	NULL	0	NULL	model antigen systems	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Researchers are now taking 2P microscopy beyond the study of model antigen systems ( e.g. ovalbumin immunization ) and are applying the technique to examine infection in vivo .
	manualset3
132798	5	406266	13	NULL	NULL	0	NULL	ovalbumin immunization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Researchers are now taking 2P microscopy beyond the study of model antigen systems ( e.g. ovalbumin immunization ) and are applying the technique to examine infection in vivo .
	manualset3
132799	6	406266	13	NULL	NULL	0	NULL	technique 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Researchers are now taking 2P microscopy beyond the study of model antigen systems ( e.g. ovalbumin immunization ) and are applying the technique to examine infection in vivo .
	manualset3
132800	7	406266	13	NULL	NULL	0	NULL	infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Researchers are now taking 2P microscopy beyond the study of model antigen systems ( e.g. ovalbumin immunization ) and are applying the technique to examine infection in vivo .
	manualset3
132801	1	406267	13	NULL	NULL	0	NULL	Researches	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Researches during the last 50 years , and the advances made in clinical sleep medicine , have lead to more effective treatments for the myriad human sleep disorders .
	manualset3
132802	2	406267	13	NULL	NULL	0	NULL	last 50 years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Researches during the last 50 years , and the advances made in clinical sleep medicine , have lead to more effective treatments for the myriad human sleep disorders .
	manualset3
132803	3	406267	13	NULL	NULL	0	NULL	advances	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Researches during the last 50 years , and the advances made in clinical sleep medicine , have lead to more effective treatments for the myriad human sleep disorders .
	manualset3
132804	4	406267	13	NULL	NULL	0	NULL	clinical sleep medicine	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Researches during the last 50 years , and the advances made in clinical sleep medicine , have lead to more effective treatments for the myriad human sleep disorders .
	manualset3
132805	5	406267	13	NULL	NULL	0	NULL	treatments	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Researches during the last 50 years , and the advances made in clinical sleep medicine , have lead to more effective treatments for the myriad human sleep disorders .
	manualset3
132806	6	406267	13	NULL	NULL	0	NULL	myriad human sleep disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Researches during the last 50 years , and the advances made in clinical sleep medicine , have lead to more effective treatments for the myriad human sleep disorders .
	manualset3
132807	1	406268	13	NULL	NULL	0	NULL	lung	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Resected lung after an abbreviated rifampin regimen .
	manualset3
132808	2	406268	13	NULL	NULL	0	NULL	rifampin regimen	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Resected lung after an abbreviated rifampin regimen .
	manualset3
132809	1	406269	13	NULL	NULL	0	NULL	Resection 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Resection of midline skull base lesions involve approaches needing extensive neurovascular manipulation .
	manualset3
132810	2	406269	13	NULL	NULL	0	NULL	midline skull base lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Resection of midline skull base lesions involve approaches needing extensive neurovascular manipulation .
	manualset3
132811	3	406269	13	NULL	NULL	0	NULL	approaches	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Resection of midline skull base lesions involve approaches needing extensive neurovascular manipulation .
	manualset3
132812	4	406269	13	NULL	NULL	0	NULL	neurovascular manipulation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Resection of midline skull base lesions involve approaches needing extensive neurovascular manipulation .
	manualset3
132813	1	406270	13	NULL	NULL	0	NULL	Reserpine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Reserpine had no effect on ( ( 3 ) H ) NE uptake in HEK-293 cells transfected with the rat NET ( 293-hNET ) , cells that lack catecholamine storage vesicles .
	manualset3
132814	2	406270	13	NULL	NULL	0	NULL	effect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reserpine had no effect on ( ( 3 ) H ) NE uptake in HEK-293 cells transfected with the rat NET ( 293-hNET ) , cells that lack catecholamine storage vesicles .
	manualset3
132815	3	406270	13	NULL	NULL	0	NULL	( ( 3 ) H ) NE uptake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reserpine had no effect on ( ( 3 ) H ) NE uptake in HEK-293 cells transfected with the rat NET ( 293-hNET ) , cells that lack catecholamine storage vesicles .
	manualset3
132816	4	406270	13	NULL	NULL	0	NULL	HEK-293 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Reserpine had no effect on ( ( 3 ) H ) NE uptake in HEK-293 cells transfected with the rat NET ( 293-hNET ) , cells that lack catecholamine storage vesicles .
	manualset3
132817	5	406270	13	NULL	NULL	0	NULL	rat NET	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Reserpine had no effect on ( ( 3 ) H ) NE uptake in HEK-293 cells transfected with the rat NET ( 293-hNET ) , cells that lack catecholamine storage vesicles .
	manualset3
132818	6	406270	13	NULL	NULL	0	NULL	293-hNET	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Reserpine had no effect on ( ( 3 ) H ) NE uptake in HEK-293 cells transfected with the rat NET ( 293-hNET ) , cells that lack catecholamine storage vesicles .
	manualset3
132819	7	406270	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Reserpine had no effect on ( ( 3 ) H ) NE uptake in HEK-293 cells transfected with the rat NET ( 293-hNET ) , cells that lack catecholamine storage vesicles .
	manualset3
132820	8	406270	13	NULL	NULL	0	NULL	lack 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reserpine had no effect on ( ( 3 ) H ) NE uptake in HEK-293 cells transfected with the rat NET ( 293-hNET ) , cells that lack catecholamine storage vesicles .
	manualset3
132821	9	406270	13	NULL	NULL	0	NULL	catecholamine storage vesicles 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Reserpine had no effect on ( ( 3 ) H ) NE uptake in HEK-293 cells transfected with the rat NET ( 293-hNET ) , cells that lack catecholamine storage vesicles .
	manualset3
132822	1	406271	13	NULL	NULL	0	NULL	Cardiac transplantation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cardiac transplantation -- light and shadow ) .
	manualset3
132823	2	406271	13	NULL	NULL	NULL	NULL	light	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Cardiac transplantation -- light and shadow ) .
	manualset3
132824	3	406271	13	NULL	NULL	0	NULL	shadow	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cardiac transplantation -- light and shadow ) .
	manualset3
132825	1	406272	13	NULL	NULL	0	NULL	Resibufogenin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Resibufogenin , cinobufagin , and bufalin are cytotoxic steroids isolated from the Chinese drug Chan ` su .
	manualset3
132826	2	406272	13	NULL	NULL	0	NULL	cinobufagin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Resibufogenin , cinobufagin , and bufalin are cytotoxic steroids isolated from the Chinese drug Chan ` su .
	manualset3
132827	3	406272	13	NULL	NULL	0	NULL	bufalin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Resibufogenin , cinobufagin , and bufalin are cytotoxic steroids isolated from the Chinese drug Chan ` su .
	manualset3
132828	4	406272	13	NULL	NULL	0	NULL	cytotoxic steroids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Resibufogenin , cinobufagin , and bufalin are cytotoxic steroids isolated from the Chinese drug Chan ` su .
	manualset3
132829	5	406272	13	NULL	NULL	0	NULL	Chinese drug Chan ` su 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Resibufogenin , cinobufagin , and bufalin are cytotoxic steroids isolated from the Chinese drug Chan ` su .
	manualset3
132830	1	406273	13	NULL	NULL	0	NULL	Resident performance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Resident performance on the Council on Resident Education in Obstetrics and Gynecology ( CREOG ) In-Training Examination : years 1996 through 2002 .
	manualset3
132831	2	406273	13	NULL	NULL	0	NULL	Council on Resident Education in Obstetrics and Gynecology ( CREOG ) 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Resident performance on the Council on Resident Education in Obstetrics and Gynecology ( CREOG ) In-Training Examination : years 1996 through 2002 .
	manualset3
132832	3	406273	13	NULL	NULL	0	NULL	In-Training Examination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Resident performance on the Council on Resident Education in Obstetrics and Gynecology ( CREOG ) In-Training Examination : years 1996 through 2002 .
	manualset3
132833	4	406273	13	NULL	NULL	NULL	NULL	years 1996 through 2002 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Resident performance on the Council on Resident Education in Obstetrics and Gynecology ( CREOG ) In-Training Examination : years 1996 through 2002 .
	manualset3
132834	1	406274	13	NULL	NULL	0	NULL	Residual normal stem cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Residual normal stem cells can be detected in newly diagnosed chronic myeloid leukemia patients by a new flow cytometric approach and predict for optimal response to imatinib .
	manualset3
132835	2	406274	13	NULL	NULL	0	NULL	chronic myeloid leukemia patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Residual normal stem cells can be detected in newly diagnosed chronic myeloid leukemia patients by a new flow cytometric approach and predict for optimal response to imatinib .
	manualset3
132836	3	406274	13	NULL	NULL	0	NULL	flow cytometric approach	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Residual normal stem cells can be detected in newly diagnosed chronic myeloid leukemia patients by a new flow cytometric approach and predict for optimal response to imatinib .
	manualset3
132837	4	406274	13	NULL	NULL	0	NULL	optimal response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Residual normal stem cells can be detected in newly diagnosed chronic myeloid leukemia patients by a new flow cytometric approach and predict for optimal response to imatinib .
	manualset3
132838	5	406274	13	NULL	NULL	0	NULL	imatinib	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Residual normal stem cells can be detected in newly diagnosed chronic myeloid leukemia patients by a new flow cytometric approach and predict for optimal response to imatinib .
	manualset3
133132	1	406275	13	NULL	NULL	0	NULL	Residual striations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Residual striations from these plunging columns persist throughout the bulk of the liquid so long as evaporation continues .
	manualset3
133133	2	406275	13	NULL	NULL	0	NULL	columns	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Residual striations from these plunging columns persist throughout the bulk of the liquid so long as evaporation continues .
	manualset3
133134	3	406275	13	NULL	NULL	0	NULL	bulk 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Residual striations from these plunging columns persist throughout the bulk of the liquid so long as evaporation continues .
	manualset3
133135	4	406275	13	NULL	NULL	0	NULL	liquid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Residual striations from these plunging columns persist throughout the bulk of the liquid so long as evaporation continues .
	manualset3
133136	5	406275	13	NULL	NULL	0	NULL	evaporation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Residual striations from these plunging columns persist throughout the bulk of the liquid so long as evaporation continues .
	manualset3
133137	1	406276	13	NULL	NULL	0	NULL	Residual viability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Residual viability within an infarct-related segment was confirmed by NH3 - and FDG-PET .
	manualset3
133138	2	406276	13	NULL	NULL	NULL	NULL	segment	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Residual viability within an infarct-related segment was confirmed by NH3 - and FDG-PET .
	manualset3
133139	3	406276	13	NULL	NULL	0	NULL	FDG-PET	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Residual viability within an infarct-related segment was confirmed by NH3 - and FDG-PET .
	manualset3
133140	4	406276	13	NULL	NULL	0	NULL	NH3-PET	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Residual viability within an infarct-related segment was confirmed by NH3 - and FDG-PET .
	manualset3
133141	1	406277	13	NULL	NULL	0	NULL	Resin films	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Resin films were prepared for transmission electron microscopy ( TEM ) after immersion in ammonical silver nitrate .
	manualset3
133142	2	406277	13	NULL	NULL	0	NULL	transmission electron microscopy ( TEM )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Resin films were prepared for transmission electron microscopy ( TEM ) after immersion in ammonical silver nitrate .
	manualset3
133143	3	406277	13	NULL	NULL	0	NULL	immersion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Resin films were prepared for transmission electron microscopy ( TEM ) after immersion in ammonical silver nitrate .
	manualset3
133144	4	406277	13	NULL	NULL	0	NULL	ammonical silver nitrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Resin films were prepared for transmission electron microscopy ( TEM ) after immersion in ammonical silver nitrate .
	manualset3
133145	1	406278	13	NULL	NULL	0	NULL	multiple-response analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A multiple-response analysis of aversive learning was conducted in human subjects .
	manualset3
133146	2	406278	13	NULL	NULL	0	NULL	learning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A multiple-response analysis of aversive learning was conducted in human subjects .
	manualset3
133147	3	406278	13	NULL	NULL	0	NULL	human subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A multiple-response analysis of aversive learning was conducted in human subjects .
	manualset3
133148	1	406279	13	NULL	NULL	0	NULL	Resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance and multidrug resistance was most common in serotype Typhimurium .
	manualset3
133149	2	406279	13	NULL	NULL	0	NULL	multidrug resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance and multidrug resistance was most common in serotype Typhimurium .
	manualset3
133150	3	406279	13	NULL	NULL	0	NULL	serotype Typhimurium	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance and multidrug resistance was most common in serotype Typhimurium .
	manualset3
133151	1	406280	13	NULL	NULL	0	NULL	Resistance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance of Bacillus subtilis spores to inactivation by gamma irradiation and heating in the presence of a bactericide .
	manualset3
133152	2	406280	13	NULL	NULL	0	NULL	Bacillus subtilis spores	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance of Bacillus subtilis spores to inactivation by gamma irradiation and heating in the presence of a bactericide .
	manualset3
133153	3	406280	13	NULL	NULL	0	NULL	inactivation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance of Bacillus subtilis spores to inactivation by gamma irradiation and heating in the presence of a bactericide .
	manualset3
133154	4	406280	13	NULL	NULL	0	NULL	gamma irradiation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance of Bacillus subtilis spores to inactivation by gamma irradiation and heating in the presence of a bactericide .
	manualset3
133155	5	406280	13	NULL	NULL	0	NULL	heating	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance of Bacillus subtilis spores to inactivation by gamma irradiation and heating in the presence of a bactericide .
	manualset3
133156	6	406280	13	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance of Bacillus subtilis spores to inactivation by gamma irradiation and heating in the presence of a bactericide .
	manualset3
133157	7	406280	13	NULL	NULL	0	NULL	bactericide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance of Bacillus subtilis spores to inactivation by gamma irradiation and heating in the presence of a bactericide .
	manualset3
133165	1	406281	13	NULL	NULL	NULL	NULL	Resistance	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Resistance to N-iodoacetylglucosamine is not absolute , and depends on the presence of glucose or certain other sugars ; there is no resistance during growth on maltose , glycerol or succinate .
	manualset3
133166	2	406281	13	NULL	NULL	0	NULL	N-iodoacetylglucosamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance to N-iodoacetylglucosamine is not absolute , and depends on the presence of glucose or certain other sugars ; there is no resistance during growth on maltose , glycerol or succinate .
	manualset3
133168	3	406281	13	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance to N-iodoacetylglucosamine is not absolute , and depends on the presence of glucose or certain other sugars ; there is no resistance during growth on maltose , glycerol or succinate .
	manualset3
133169	4	406281	13	NULL	NULL	0	NULL	glucose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance to N-iodoacetylglucosamine is not absolute , and depends on the presence of glucose or certain other sugars ; there is no resistance during growth on maltose , glycerol or succinate .
	manualset3
133171	5	406281	13	NULL	NULL	0	NULL	sugars	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance to N-iodoacetylglucosamine is not absolute , and depends on the presence of glucose or certain other sugars ; there is no resistance during growth on maltose , glycerol or succinate .
	manualset3
133172	6	406281	13	NULL	NULL	NULL	NULL	resistance 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Resistance to N-iodoacetylglucosamine is not absolute , and depends on the presence of glucose or certain other sugars ; there is no resistance during growth on maltose , glycerol or succinate .
	manualset3
133173	7	406281	13	NULL	NULL	0	NULL	growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance to N-iodoacetylglucosamine is not absolute , and depends on the presence of glucose or certain other sugars ; there is no resistance during growth on maltose , glycerol or succinate .
	manualset3
133174	8	406281	13	NULL	NULL	0	NULL	maltose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance to N-iodoacetylglucosamine is not absolute , and depends on the presence of glucose or certain other sugars ; there is no resistance during growth on maltose , glycerol or succinate .
	manualset3
133175	9	406281	13	NULL	NULL	0	NULL	glycerol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance to N-iodoacetylglucosamine is not absolute , and depends on the presence of glucose or certain other sugars ; there is no resistance during growth on maltose , glycerol or succinate .
	manualset3
133176	10	406281	13	NULL	NULL	0	NULL	succinate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance to N-iodoacetylglucosamine is not absolute , and depends on the presence of glucose or certain other sugars ; there is no resistance during growth on maltose , glycerol or succinate .
	manualset3
133180	1	406282	13	NULL	NULL	0	NULL	Resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance to Pst ( avrPto ) in 96T133-3 was inherited as a single dominant locus and cosegregated with a restriction fragment length polymorphism detected by the Pto gene .
	manualset3
133187	2	406282	13	NULL	NULL	0	NULL	Pst 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance to Pst ( avrPto ) in 96T133-3 was inherited as a single dominant locus and cosegregated with a restriction fragment length polymorphism detected by the Pto gene .
	manualset3
133188	3	406282	13	NULL	NULL	0	NULL	avrPto	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance to Pst ( avrPto ) in 96T133-3 was inherited as a single dominant locus and cosegregated with a restriction fragment length polymorphism detected by the Pto gene .
	manualset3
133193	4	406282	13	NULL	NULL	0	NULL	96T133-3	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance to Pst ( avrPto ) in 96T133-3 was inherited as a single dominant locus and cosegregated with a restriction fragment length polymorphism detected by the Pto gene .
	manualset3
133198	5	406282	13	NULL	NULL	0	NULL	single dominant locus	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance to Pst ( avrPto ) in 96T133-3 was inherited as a single dominant locus and cosegregated with a restriction fragment length polymorphism detected by the Pto gene .
	manualset3
133200	6	406282	13	NULL	NULL	0	NULL	restriction fragment length polymorphism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance to Pst ( avrPto ) in 96T133-3 was inherited as a single dominant locus and cosegregated with a restriction fragment length polymorphism detected by the Pto gene .
	manualset3
133202	7	406282	13	NULL	NULL	0	NULL	Pto gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance to Pst ( avrPto ) in 96T133-3 was inherited as a single dominant locus and cosegregated with a restriction fragment length polymorphism detected by the Pto gene .
	manualset3
133208	1	406283	13	NULL	NULL	0	NULL	Resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance to chemotherapy by some human tumors may be due to overexpression of membrane-associated transport proteins .
	manualset3
133209	2	406283	13	NULL	NULL	0	NULL	chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance to chemotherapy by some human tumors may be due to overexpression of membrane-associated transport proteins .
	manualset3
133211	3	406283	13	NULL	NULL	0	NULL	human tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance to chemotherapy by some human tumors may be due to overexpression of membrane-associated transport proteins .
	manualset3
133213	4	406283	13	NULL	NULL	0	NULL	overexpression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance to chemotherapy by some human tumors may be due to overexpression of membrane-associated transport proteins .
	manualset3
133215	5	406283	13	NULL	NULL	0	NULL	membrane-associated transport proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance to chemotherapy by some human tumors may be due to overexpression of membrane-associated transport proteins .
	manualset3
133216	1	406284	13	NULL	NULL	0	NULL	Resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance to endocrine therapy in breast cancer : exploiting estrogen receptor/growth factor signaling crosstalk .
	manualset3
133217	2	406284	13	NULL	NULL	0	NULL	endocrine therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance to endocrine therapy in breast cancer : exploiting estrogen receptor/growth factor signaling crosstalk .
	manualset3
133218	3	406284	13	NULL	NULL	0	NULL	breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance to endocrine therapy in breast cancer : exploiting estrogen receptor/growth factor signaling crosstalk .
	manualset3
133222	4	406284	13	NULL	NULL	0	NULL	estrogen receptor/growth factor signaling crosstalk 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Resistance to endocrine therapy in breast cancer : exploiting estrogen receptor/growth factor signaling crosstalk .
	manualset3
133224	1	406285	13	NULL	NULL	NULL	NULL	Resolution 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Resolution of sick building syndrome in a high-security facility .
	manualset3
133226	2	406285	13	NULL	NULL	0	NULL	sick building syndrome 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Resolution of sick building syndrome in a high-security facility .
	manualset3
133231	3	406285	13	NULL	NULL	0	NULL	high-security facility	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Resolution of sick building syndrome in a high-security facility .
	manualset3
133232	1	406286	13	NULL	NULL	0	NULL	Resolving powers ( FWHH )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Resolving powers ( FWHH ) as high as 1.7 x 10 ( 7 ) for the ( M + H ) ( + ) of vasopressin at m/z 1084.5 in a 7.0-tesla induction can be obtained when using trap compensation .
	manualset3
133234	2	406286	13	NULL	NULL	0	NULL	1.7 x 10 ( 7 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Resolving powers ( FWHH ) as high as 1.7 x 10 ( 7 ) for the ( M + H ) ( + ) of vasopressin at m/z 1084.5 in a 7.0-tesla induction can be obtained when using trap compensation .
	manualset3
133245	3	406286	13	NULL	NULL	0	NULL	 ( M + H ) ( + ) of vasopressin	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Resolving powers ( FWHH ) as high as 1.7 x 10 ( 7 ) for the ( M + H ) ( + ) of vasopressin at m/z 1084.5 in a 7.0-tesla induction can be obtained when using trap compensation .
	manualset3
133246	4	406286	13	NULL	NULL	0	NULL	m/z 1084.5 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Resolving powers ( FWHH ) as high as 1.7 x 10 ( 7 ) for the ( M + H ) ( + ) of vasopressin at m/z 1084.5 in a 7.0-tesla induction can be obtained when using trap compensation .
	manualset3
133247	5	406286	13	NULL	NULL	0	NULL	7.0-tesla	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Resolving powers ( FWHH ) as high as 1.7 x 10 ( 7 ) for the ( M + H ) ( + ) of vasopressin at m/z 1084.5 in a 7.0-tesla induction can be obtained when using trap compensation .
	manualset3
133248	6	406286	13	NULL	NULL	0	NULL	induction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Resolving powers ( FWHH ) as high as 1.7 x 10 ( 7 ) for the ( M + H ) ( + ) of vasopressin at m/z 1084.5 in a 7.0-tesla induction can be obtained when using trap compensation .
	manualset3
133249	7	406286	13	NULL	NULL	0	NULL	trap compensation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Resolving powers ( FWHH ) as high as 1.7 x 10 ( 7 ) for the ( M + H ) ( + ) of vasopressin at m/z 1084.5 in a 7.0-tesla induction can be obtained when using trap compensation .
	manualset3
133252	1	406287	13	NULL	NULL	0	NULL	Resonances	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Resonances of Trp3 and Tyr69 protons of the two proteins were assigned .
	manualset3
133256	2	406287	13	NULL	NULL	0	NULL	Trp3 protons	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Resonances of Trp3 and Tyr69 protons of the two proteins were assigned .
	manualset3
133257	3	406287	13	NULL	NULL	0	NULL	Tyr69 protons	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Resonances of Trp3 and Tyr69 protons of the two proteins were assigned .
	manualset3
133258	4	406287	13	NULL	NULL	0	NULL	two proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Resonances of Trp3 and Tyr69 protons of the two proteins were assigned .
	manualset3
133271	1	406288	13	NULL	NULL	0	NULL	multistage analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A multistage analysis and Oaxaca-Blinder decomposition are used to explore the sources of racial disparities in health .
	manualset3
133272	2	406288	13	NULL	NULL	0	NULL	Oaxaca-Blinder decomposition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A multistage analysis and Oaxaca-Blinder decomposition are used to explore the sources of racial disparities in health .
	manualset3
133274	3	406288	13	NULL	NULL	0	NULL	sources	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A multistage analysis and Oaxaca-Blinder decomposition are used to explore the sources of racial disparities in health .
	manualset3
133276	4	406288	13	NULL	NULL	0	NULL	racial disparities 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A multistage analysis and Oaxaca-Blinder decomposition are used to explore the sources of racial disparities in health .
	manualset3
133279	5	406288	13	NULL	NULL	0	NULL	health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A multistage analysis and Oaxaca-Blinder decomposition are used to explore the sources of racial disparities in health .
	manualset3
133282	1	406289	13	NULL	NULL	0	NULL	Resonant frequency	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Resonant frequency and frequency dependence of resistance correlated significantly with selected parameters of the forced expiratory flow volume curve : correlation coefficient values ranged from 0.492 between frequency dependence and FVC and 0.668 between resonant frequency and FEV1 .
	manualset3
133284	2	406289	13	NULL	NULL	0	NULL	frequency dependence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Resonant frequency and frequency dependence of resistance correlated significantly with selected parameters of the forced expiratory flow volume curve : correlation coefficient values ranged from 0.492 between frequency dependence and FVC and 0.668 between resonant frequency and FEV1 .
	manualset3
133286	3	406289	13	NULL	NULL	NULL	NULL	resistance	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Resonant frequency and frequency dependence of resistance correlated significantly with selected parameters of the forced expiratory flow volume curve : correlation coefficient values ranged from 0.492 between frequency dependence and FVC and 0.668 between resonant frequency and FEV1 .
	manualset3
133288	4	406289	13	NULL	NULL	0	NULL	parameters	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Resonant frequency and frequency dependence of resistance correlated significantly with selected parameters of the forced expiratory flow volume curve : correlation coefficient values ranged from 0.492 between frequency dependence and FVC and 0.668 between resonant frequency and FEV1 .
	manualset3
133291	5	406289	13	NULL	NULL	0	NULL	forced expiratory flow volume curve	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Resonant frequency and frequency dependence of resistance correlated significantly with selected parameters of the forced expiratory flow volume curve : correlation coefficient values ranged from 0.492 between frequency dependence and FVC and 0.668 between resonant frequency and FEV1 .
	manualset3
133292	6	406289	13	NULL	NULL	0	NULL	correlation coefficient values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Resonant frequency and frequency dependence of resistance correlated significantly with selected parameters of the forced expiratory flow volume curve : correlation coefficient values ranged from 0.492 between frequency dependence and FVC and 0.668 between resonant frequency and FEV1 .
	manualset3
133293	7	406289	13	NULL	NULL	0	NULL	0.492 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Resonant frequency and frequency dependence of resistance correlated significantly with selected parameters of the forced expiratory flow volume curve : correlation coefficient values ranged from 0.492 between frequency dependence and FVC and 0.668 between resonant frequency and FEV1 .
	manualset3
133295	8	406289	13	NULL	NULL	0	NULL	frequency dependence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Resonant frequency and frequency dependence of resistance correlated significantly with selected parameters of the forced expiratory flow volume curve : correlation coefficient values ranged from 0.492 between frequency dependence and FVC and 0.668 between resonant frequency and FEV1 .
	manualset3
133298	9	406289	13	NULL	NULL	0	NULL	FVC	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Resonant frequency and frequency dependence of resistance correlated significantly with selected parameters of the forced expiratory flow volume curve : correlation coefficient values ranged from 0.492 between frequency dependence and FVC and 0.668 between resonant frequency and FEV1 .
	manualset3
133300	10	406289	13	NULL	NULL	0	NULL	0.668	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Resonant frequency and frequency dependence of resistance correlated significantly with selected parameters of the forced expiratory flow volume curve : correlation coefficient values ranged from 0.492 between frequency dependence and FVC and 0.668 between resonant frequency and FEV1 .
	manualset3
133301	11	406289	13	NULL	NULL	0	NULL	resonant frequency	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Resonant frequency and frequency dependence of resistance correlated significantly with selected parameters of the forced expiratory flow volume curve : correlation coefficient values ranged from 0.492 between frequency dependence and FVC and 0.668 between resonant frequency and FEV1 .
	manualset3
133303	12	406289	13	NULL	NULL	0	NULL	 FEV1 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Resonant frequency and frequency dependence of resistance correlated significantly with selected parameters of the forced expiratory flow volume curve : correlation coefficient values ranged from 0.492 between frequency dependence and FVC and 0.668 between resonant frequency and FEV1 .
	manualset3
133306	1	406290	13	NULL	NULL	0	NULL	Resource allocation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Resource allocation and budgetary mechanisms for decentralized health systems : experiences from Balochistan , Pakistan .
	manualset3
133307	2	406290	13	NULL	NULL	0	NULL	budgetary mechanisms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Resource allocation and budgetary mechanisms for decentralized health systems : experiences from Balochistan , Pakistan .
	manualset3
133308	3	406290	13	NULL	NULL	NULL	NULL	health systems	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Resource allocation and budgetary mechanisms for decentralized health systems : experiences from Balochistan , Pakistan .
	manualset3
133309	4	406290	13	NULL	NULL	0	NULL	experiences	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Resource allocation and budgetary mechanisms for decentralized health systems : experiences from Balochistan , Pakistan .
	manualset3
133310	5	406290	13	NULL	NULL	0	NULL	Balochistan	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Resource allocation and budgetary mechanisms for decentralized health systems : experiences from Balochistan , Pakistan .
	manualset3
133311	6	406290	13	NULL	NULL	0	NULL	Pakistan	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Resource allocation and budgetary mechanisms for decentralized health systems : experiences from Balochistan , Pakistan .
	manualset3
133312	1	406291	13	NULL	NULL	0	NULL	Resources	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Resources are also included that allow resolution assessment by cross-validation ( NLOO2D ) ; denoising and interpretation ; and the extraction , mutual alignment , and averaging of tomographic sub-volumes .
	manualset3
133315	2	406291	13	NULL	NULL	0	NULL	resolution assessment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Resources are also included that allow resolution assessment by cross-validation ( NLOO2D ) ; denoising and interpretation ; and the extraction , mutual alignment , and averaging of tomographic sub-volumes .
	manualset3
133316	3	406291	13	NULL	NULL	0	NULL	cross-validation ( NLOO2D )	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Resources are also included that allow resolution assessment by cross-validation ( NLOO2D ) ; denoising and interpretation ; and the extraction , mutual alignment , and averaging of tomographic sub-volumes .
	manualset3
133317	4	406291	13	NULL	NULL	0	NULL	interpretation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Resources are also included that allow resolution assessment by cross-validation ( NLOO2D ) ; denoising and interpretation ; and the extraction , mutual alignment , and averaging of tomographic sub-volumes .
	manualset3
133318	5	406291	13	NULL	NULL	0	NULL	extraction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Resources are also included that allow resolution assessment by cross-validation ( NLOO2D ) ; denoising and interpretation ; and the extraction , mutual alignment , and averaging of tomographic sub-volumes .
	manualset3
133319	6	406291	13	NULL	NULL	0	NULL	mutual alignment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Resources are also included that allow resolution assessment by cross-validation ( NLOO2D ) ; denoising and interpretation ; and the extraction , mutual alignment , and averaging of tomographic sub-volumes .
	manualset3
133321	7	406291	13	NULL	NULL	0	NULL	 tomographic sub-volumes	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Resources are also included that allow resolution assessment by cross-validation ( NLOO2D ) ; denoising and interpretation ; and the extraction , mutual alignment , and averaging of tomographic sub-volumes .
	manualset3
134891	8	406291	13	NULL	NULL	0	NULL	denoising	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Resources are also included that allow resolution assessment by cross-validation ( NLOO2D ) ; denoising and interpretation ; and the extraction , mutual alignment , and averaging of tomographic sub-volumes .
	manualset3
134892	9	406291	13	NULL	NULL	0	NULL	averaging	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Resources are also included that allow resolution assessment by cross-validation ( NLOO2D ) ; denoising and interpretation ; and the extraction , mutual alignment , and averaging of tomographic sub-volumes .
	manualset3
133323	1	406292	13	NULL	NULL	0	NULL	Respect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Respect for the dignity and sanctity of human life , and a duty to preserve health , are grounded in biblical and legal traditions and are the basis of contemporary Jewish responses to such issues as abortion , contraception , euthanasia , and organ transplantation .
	manualset3
133324	2	406292	13	NULL	NULL	0	NULL	dignity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Respect for the dignity and sanctity of human life , and a duty to preserve health , are grounded in biblical and legal traditions and are the basis of contemporary Jewish responses to such issues as abortion , contraception , euthanasia , and organ transplantation .
	manualset3
133325	3	406292	13	NULL	NULL	0	NULL	sanctity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Respect for the dignity and sanctity of human life , and a duty to preserve health , are grounded in biblical and legal traditions and are the basis of contemporary Jewish responses to such issues as abortion , contraception , euthanasia , and organ transplantation .
	manualset3
133326	4	406292	13	NULL	NULL	NULL	NULL	human life	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Respect for the dignity and sanctity of human life , and a duty to preserve health , are grounded in biblical and legal traditions and are the basis of contemporary Jewish responses to such issues as abortion , contraception , euthanasia , and organ transplantation .
	manualset3
133327	5	406292	13	NULL	NULL	0	NULL	duty	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Respect for the dignity and sanctity of human life , and a duty to preserve health , are grounded in biblical and legal traditions and are the basis of contemporary Jewish responses to such issues as abortion , contraception , euthanasia , and organ transplantation .
	manualset3
133328	6	406292	13	NULL	NULL	0	NULL	health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Respect for the dignity and sanctity of human life , and a duty to preserve health , are grounded in biblical and legal traditions and are the basis of contemporary Jewish responses to such issues as abortion , contraception , euthanasia , and organ transplantation .
	manualset3
133329	7	406292	13	NULL	NULL	0	NULL	biblical traditions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Respect for the dignity and sanctity of human life , and a duty to preserve health , are grounded in biblical and legal traditions and are the basis of contemporary Jewish responses to such issues as abortion , contraception , euthanasia , and organ transplantation .
	manualset3
133330	8	406292	13	NULL	NULL	0	NULL	legal traditions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Respect for the dignity and sanctity of human life , and a duty to preserve health , are grounded in biblical and legal traditions and are the basis of contemporary Jewish responses to such issues as abortion , contraception , euthanasia , and organ transplantation .
	manualset3
133331	9	406292	13	NULL	NULL	0	NULL	basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Respect for the dignity and sanctity of human life , and a duty to preserve health , are grounded in biblical and legal traditions and are the basis of contemporary Jewish responses to such issues as abortion , contraception , euthanasia , and organ transplantation .
	manualset3
133332	10	406292	13	NULL	NULL	0	NULL	contemporary Jewish responses	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Respect for the dignity and sanctity of human life , and a duty to preserve health , are grounded in biblical and legal traditions and are the basis of contemporary Jewish responses to such issues as abortion , contraception , euthanasia , and organ transplantation .
	manualset3
133333	11	406292	13	NULL	NULL	0	NULL	issues	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Respect for the dignity and sanctity of human life , and a duty to preserve health , are grounded in biblical and legal traditions and are the basis of contemporary Jewish responses to such issues as abortion , contraception , euthanasia , and organ transplantation .
	manualset3
133334	12	406292	13	NULL	NULL	0	NULL	abortion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Respect for the dignity and sanctity of human life , and a duty to preserve health , are grounded in biblical and legal traditions and are the basis of contemporary Jewish responses to such issues as abortion , contraception , euthanasia , and organ transplantation .
	manualset3
133335	13	406292	13	NULL	NULL	0	NULL	contraception	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Respect for the dignity and sanctity of human life , and a duty to preserve health , are grounded in biblical and legal traditions and are the basis of contemporary Jewish responses to such issues as abortion , contraception , euthanasia , and organ transplantation .
	manualset3
133336	14	406292	13	NULL	NULL	0	NULL	euthanasia 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Respect for the dignity and sanctity of human life , and a duty to preserve health , are grounded in biblical and legal traditions and are the basis of contemporary Jewish responses to such issues as abortion , contraception , euthanasia , and organ transplantation .
	manualset3
133337	15	406292	13	NULL	NULL	0	NULL	organ transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Respect for the dignity and sanctity of human life , and a duty to preserve health , are grounded in biblical and legal traditions and are the basis of contemporary Jewish responses to such issues as abortion , contraception , euthanasia , and organ transplantation .
	manualset3
133338	1	406293	13	NULL	NULL	0	NULL	Respirations 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Respirations were measured by single chamber plethysmograph , and blood pressure and heart period were transduced by a telemetric implant .
	manualset3
133339	2	406293	13	NULL	NULL	0	NULL	single chamber plethysmograph	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Respirations were measured by single chamber plethysmograph , and blood pressure and heart period were transduced by a telemetric implant .
	manualset3
133340	3	406293	13	NULL	NULL	0	NULL	blood pressure 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Respirations were measured by single chamber plethysmograph , and blood pressure and heart period were transduced by a telemetric implant .
	manualset3
133341	4	406293	13	NULL	NULL	0	NULL	heart period 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Respirations were measured by single chamber plethysmograph , and blood pressure and heart period were transduced by a telemetric implant .
	manualset3
133342	5	406293	13	NULL	NULL	0	NULL	telemetric implant	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Respirations were measured by single chamber plethysmograph , and blood pressure and heart period were transduced by a telemetric implant .
	manualset3
133343	1	406294	13	NULL	NULL	0	NULL	Respiratory parameters	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Respiratory and hemodynamic parameters and ICP ( epidural probe ) were continuously monitored and recorded on an integrated data bank .
	manualset3
133344	2	406294	13	NULL	NULL	0	NULL	hemodynamic parameters	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Respiratory and hemodynamic parameters and ICP ( epidural probe ) were continuously monitored and recorded on an integrated data bank .
	manualset3
133345	3	406294	13	NULL	NULL	0	NULL	ICP ( epidural probe )	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Respiratory and hemodynamic parameters and ICP ( epidural probe ) were continuously monitored and recorded on an integrated data bank .
	manualset3
133346	4	406294	13	NULL	NULL	NULL	NULL	data bank	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Respiratory and hemodynamic parameters and ICP ( epidural probe ) were continuously monitored and recorded on an integrated data bank .
	manualset3
133347	1	406295	13	NULL	NULL	0	NULL	Respiratory effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Respiratory effects of 5 ' - ethylcarboxamidoadenosine , an analog of adenosine , following microinjections into the nucleus tractus solitarius of rats .
	manualset3
133348	2	406295	13	NULL	NULL	0	NULL	5 ' - ethylcarboxamidoadenosine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Respiratory effects of 5 ' - ethylcarboxamidoadenosine , an analog of adenosine , following microinjections into the nucleus tractus solitarius of rats .
	manualset3
133349	3	406295	13	NULL	NULL	0	NULL	analog of adenosine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Respiratory effects of 5 ' - ethylcarboxamidoadenosine , an analog of adenosine , following microinjections into the nucleus tractus solitarius of rats .
	manualset3
133350	4	406295	13	NULL	NULL	0	NULL	microinjections	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Respiratory effects of 5 ' - ethylcarboxamidoadenosine , an analog of adenosine , following microinjections into the nucleus tractus solitarius of rats .
	manualset3
133351	5	406295	13	NULL	NULL	0	NULL	nucleus tractus solitarius	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Respiratory effects of 5 ' - ethylcarboxamidoadenosine , an analog of adenosine , following microinjections into the nucleus tractus solitarius of rats .
	manualset3
133352	6	406295	13	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Respiratory effects of 5 ' - ethylcarboxamidoadenosine , an analog of adenosine , following microinjections into the nucleus tractus solitarius of rats .
	manualset3
133355	1	406296	13	NULL	NULL	0	NULL	Respiratory failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Respiratory failure is a major cause of mortality during septic shock and is due in part to decreased ventilatory muscle contraction .
	manualset3
133356	2	406296	13	NULL	NULL	0	NULL	major cause 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Respiratory failure is a major cause of mortality during septic shock and is due in part to decreased ventilatory muscle contraction .
	manualset3
133357	3	406296	13	NULL	NULL	0	NULL	mortality 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Respiratory failure is a major cause of mortality during septic shock and is due in part to decreased ventilatory muscle contraction .
	manualset3
133358	4	406296	13	NULL	NULL	0	NULL	septic shock	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Respiratory failure is a major cause of mortality during septic shock and is due in part to decreased ventilatory muscle contraction .
	manualset3
133359	5	406296	13	NULL	NULL	0	NULL	ventilatory muscle contraction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Respiratory failure is a major cause of mortality during septic shock and is due in part to decreased ventilatory muscle contraction .
	manualset3
133360	1	406297	13	NULL	NULL	0	NULL	Respiratory viruses 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Respiratory viruses promote bacterial adhesion to respiratory epithelial cells , a process that may increase bacterial colonization and contribute to disease .
	manualset3
133361	2	406297	13	NULL	NULL	0	NULL	bacterial adhesion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Respiratory viruses promote bacterial adhesion to respiratory epithelial cells , a process that may increase bacterial colonization and contribute to disease .
	manualset3
133362	3	406297	13	NULL	NULL	0	NULL	respiratory epithelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Respiratory viruses promote bacterial adhesion to respiratory epithelial cells , a process that may increase bacterial colonization and contribute to disease .
	manualset3
133363	4	406297	13	NULL	NULL	0	NULL	process	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Respiratory viruses promote bacterial adhesion to respiratory epithelial cells , a process that may increase bacterial colonization and contribute to disease .
	manualset3
133364	5	406297	13	NULL	NULL	0	NULL	bacterial colonization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Respiratory viruses promote bacterial adhesion to respiratory epithelial cells , a process that may increase bacterial colonization and contribute to disease .
	manualset3
133365	6	406297	13	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Respiratory viruses promote bacterial adhesion to respiratory epithelial cells , a process that may increase bacterial colonization and contribute to disease .
	manualset3
133366	1	406298	13	NULL	NULL	0	NULL	Responding 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Responding to women 's needs .
	manualset3
133367	2	406298	13	NULL	NULL	0	NULL	women 's needs	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Responding to women 's needs .
	manualset3
133370	1	406299	13	NULL	NULL	0	NULL	Response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Response , defined as a reduction in the concentration of the M-component in serum or urine , was observed in 58 % of patients , and a clearly defined plateau phase was noted in 38 % of the cases .
	manualset3
133371	2	406299	13	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Response , defined as a reduction in the concentration of the M-component in serum or urine , was observed in 58 % of patients , and a clearly defined plateau phase was noted in 38 % of the cases .
	manualset3
133372	3	406299	13	NULL	NULL	0	NULL	concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Response , defined as a reduction in the concentration of the M-component in serum or urine , was observed in 58 % of patients , and a clearly defined plateau phase was noted in 38 % of the cases .
	manualset3
133374	4	406299	13	NULL	NULL	0	NULL	M-component 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Response , defined as a reduction in the concentration of the M-component in serum or urine , was observed in 58 % of patients , and a clearly defined plateau phase was noted in 38 % of the cases .
	manualset3
133375	5	406299	13	NULL	NULL	NULL	NULL	serum	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Response , defined as a reduction in the concentration of the M-component in serum or urine , was observed in 58 % of patients , and a clearly defined plateau phase was noted in 38 % of the cases .
	manualset3
133376	6	406299	13	NULL	NULL	0	NULL	urine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Response , defined as a reduction in the concentration of the M-component in serum or urine , was observed in 58 % of patients , and a clearly defined plateau phase was noted in 38 % of the cases .
	manualset3
133377	7	406299	13	NULL	NULL	0	NULL	58 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Response , defined as a reduction in the concentration of the M-component in serum or urine , was observed in 58 % of patients , and a clearly defined plateau phase was noted in 38 % of the cases .
	manualset3
133378	8	406299	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Response , defined as a reduction in the concentration of the M-component in serum or urine , was observed in 58 % of patients , and a clearly defined plateau phase was noted in 38 % of the cases .
	manualset3
133379	9	406299	13	NULL	NULL	NULL	NULL	plateau phase	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Response , defined as a reduction in the concentration of the M-component in serum or urine , was observed in 58 % of patients , and a clearly defined plateau phase was noted in 38 % of the cases .
	manualset3
133381	10	406299	13	NULL	NULL	0	NULL	38 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Response , defined as a reduction in the concentration of the M-component in serum or urine , was observed in 58 % of patients , and a clearly defined plateau phase was noted in 38 % of the cases .
	manualset3
133383	11	406299	13	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Response , defined as a reduction in the concentration of the M-component in serum or urine , was observed in 58 % of patients , and a clearly defined plateau phase was noted in 38 % of the cases .
	manualset3
133392	1	406300	13	NULL	NULL	NULL	NULL	Response 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Response of cholesterol synthesis to cholesterol feeding in men with different apolipoprotein E genotypes .
	manualset3
133394	2	406300	13	NULL	NULL	0	NULL	cholesterol synthesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Response of cholesterol synthesis to cholesterol feeding in men with different apolipoprotein E genotypes .
	manualset3
133398	3	406300	13	NULL	NULL	NULL	NULL	cholesterol feeding	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Response of cholesterol synthesis to cholesterol feeding in men with different apolipoprotein E genotypes .
	manualset3
133400	4	406300	13	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Response of cholesterol synthesis to cholesterol feeding in men with different apolipoprotein E genotypes .
	manualset3
133402	5	406300	13	NULL	NULL	0	NULL	apolipoprotein E genotypes 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Response of cholesterol synthesis to cholesterol feeding in men with different apolipoprotein E genotypes .
	manualset3
133569	1	406301	13	NULL	NULL	0	NULL	Response 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Response of maternally isolated rock pigeons ( Columba livia domestica ) to different dietary concentrations of mannan-oligosaccharide .
	manualset3
133570	2	406301	13	NULL	NULL	0	NULL	maternally isolated rock pigeons 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Response of maternally isolated rock pigeons ( Columba livia domestica ) to different dietary concentrations of mannan-oligosaccharide .
	manualset3
133571	3	406301	13	NULL	NULL	0	NULL	Columba livia domestica	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Response of maternally isolated rock pigeons ( Columba livia domestica ) to different dietary concentrations of mannan-oligosaccharide .
	manualset3
133572	4	406301	13	NULL	NULL	0	NULL	dietary concentrations 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Response of maternally isolated rock pigeons ( Columba livia domestica ) to different dietary concentrations of mannan-oligosaccharide .
	manualset3
133573	5	406301	13	NULL	NULL	0	NULL	mannan-oligosaccharide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Response of maternally isolated rock pigeons ( Columba livia domestica ) to different dietary concentrations of mannan-oligosaccharide .
	manualset3
133574	1	406302	13	NULL	NULL	0	NULL	Response 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Response of pial arterioles to nitroglycerin was similar in nonalcohol-fed and alcohol-fed rats , and was not affected by apocynin .
	manualset3
133575	2	406302	13	NULL	NULL	NULL	NULL	pial arterioles 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Response of pial arterioles to nitroglycerin was similar in nonalcohol-fed and alcohol-fed rats , and was not affected by apocynin .
	manualset3
133576	3	406302	13	NULL	NULL	0	NULL	nitroglycerin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Response of pial arterioles to nitroglycerin was similar in nonalcohol-fed and alcohol-fed rats , and was not affected by apocynin .
	manualset3
133577	4	406302	13	NULL	NULL	0	NULL	nonalcohol-fed rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Response of pial arterioles to nitroglycerin was similar in nonalcohol-fed and alcohol-fed rats , and was not affected by apocynin .
	manualset3
133578	5	406302	13	NULL	NULL	0	NULL	alcohol-fed rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Response of pial arterioles to nitroglycerin was similar in nonalcohol-fed and alcohol-fed rats , and was not affected by apocynin .
	manualset3
133579	6	406302	13	NULL	NULL	0	NULL	apocynin 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Response of pial arterioles to nitroglycerin was similar in nonalcohol-fed and alcohol-fed rats , and was not affected by apocynin .
	manualset3
133580	1	406303	13	NULL	NULL	0	NULL	Response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Response of psoriasis to red laser light ( 630 nm ) following systemic injection of hematoporphyrin derivative .
	manualset3
133581	2	406303	13	NULL	NULL	0	NULL	psoriasis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Response of psoriasis to red laser light ( 630 nm ) following systemic injection of hematoporphyrin derivative .
	manualset3
133582	3	406303	13	NULL	NULL	0	NULL	red laser light 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Response of psoriasis to red laser light ( 630 nm ) following systemic injection of hematoporphyrin derivative .
	manualset3
133583	4	406303	13	NULL	NULL	0	NULL	630 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Response of psoriasis to red laser light ( 630 nm ) following systemic injection of hematoporphyrin derivative .
	manualset3
133584	5	406303	13	NULL	NULL	0	NULL	systemic injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Response of psoriasis to red laser light ( 630 nm ) following systemic injection of hematoporphyrin derivative .
	manualset3
133585	6	406303	13	NULL	NULL	0	NULL	hematoporphyrin derivative	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Response of psoriasis to red laser light ( 630 nm ) following systemic injection of hematoporphyrin derivative .
	manualset3
133586	1	406304	13	NULL	NULL	0	NULL	Response 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Response of sulfate-reducing bacteria to an artificial oil-spill in a coastal marine sediment .
	manualset3
133587	2	406304	13	NULL	NULL	0	NULL	 sulfate-reducing bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Response of sulfate-reducing bacteria to an artificial oil-spill in a coastal marine sediment .
	manualset3
133588	3	406304	13	NULL	NULL	0	NULL	artificial oil-spill 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Response of sulfate-reducing bacteria to an artificial oil-spill in a coastal marine sediment .
	manualset3
133589	4	406304	13	NULL	NULL	0	NULL	coastal marine sediment	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Response of sulfate-reducing bacteria to an artificial oil-spill in a coastal marine sediment .
	manualset3
133590	1	406305	13	NULL	NULL	0	NULL	multivariate analysis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A multivariate analysis of survival showed disease stage , hemoglobin level , histologic grade , and total dose to be significant factors in outcome .
	manualset3
133591	2	406305	13	NULL	NULL	0	NULL	survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A multivariate analysis of survival showed disease stage , hemoglobin level , histologic grade , and total dose to be significant factors in outcome .
	manualset3
133592	3	406305	13	NULL	NULL	0	NULL	disease stage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A multivariate analysis of survival showed disease stage , hemoglobin level , histologic grade , and total dose to be significant factors in outcome .
	manualset3
133593	4	406305	13	NULL	NULL	0	NULL	hemoglobin level	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A multivariate analysis of survival showed disease stage , hemoglobin level , histologic grade , and total dose to be significant factors in outcome .
	manualset3
133594	5	406305	13	NULL	NULL	0	NULL	histologic grade 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A multivariate analysis of survival showed disease stage , hemoglobin level , histologic grade , and total dose to be significant factors in outcome .
	manualset3
133595	6	406305	13	NULL	NULL	0	NULL	total dose	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A multivariate analysis of survival showed disease stage , hemoglobin level , histologic grade , and total dose to be significant factors in outcome .
	manualset3
133596	7	406305	13	NULL	NULL	0	NULL	significant factors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A multivariate analysis of survival showed disease stage , hemoglobin level , histologic grade , and total dose to be significant factors in outcome .
	manualset3
133597	8	406305	13	NULL	NULL	0	NULL	outcome 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A multivariate analysis of survival showed disease stage , hemoglobin level , histologic grade , and total dose to be significant factors in outcome .
	manualset3
133598	1	406306	13	NULL	NULL	0	NULL	Response timing 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Response timing and development : fixed-interval performance in precociously weaned rats .
	manualset3
133599	2	406306	13	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Response timing and development : fixed-interval performance in precociously weaned rats .
	manualset3
133600	3	406306	13	NULL	NULL	0	NULL	fixed-interval performance 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Response timing and development : fixed-interval performance in precociously weaned rats .
	manualset3
133601	4	406306	13	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Response timing and development : fixed-interval performance in precociously weaned rats .
	manualset3
133602	1	406307	13	NULL	NULL	0	NULL	Response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Response to combined cholestyramine and lovastatin therapy ) .
	manualset3
133603	2	406307	13	NULL	NULL	0	NULL	cholestyramine therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Response to combined cholestyramine and lovastatin therapy ) .
	manualset3
133604	3	406307	13	NULL	NULL	0	NULL	lovastatin therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Response to combined cholestyramine and lovastatin therapy ) .
	manualset3
133605	1	406308	13	NULL	NULL	0	NULL	Response	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Response to editorial on antioxidant therapy for chronic heart failure .
	manualset3
133606	2	406308	13	NULL	NULL	0	NULL	editorial 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Response to editorial on antioxidant therapy for chronic heart failure .
	manualset3
133607	3	406308	13	NULL	NULL	0	NULL	antioxidant therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Response to editorial on antioxidant therapy for chronic heart failure .
	manualset3
133608	4	406308	13	NULL	NULL	0	NULL	chronic heart failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Response to editorial on antioxidant therapy for chronic heart failure .
	manualset3
133609	1	406309	13	NULL	NULL	0	NULL	Responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Responses of isolated , 60 mmHg ` pressurized ' segments of the distal caudal artery of adult and juvenile Wistar rats to melatonin and the selective alpha 2-adrenoceptor agonist 5-bromo-6 - ( 2-imidazolin-2-ylamino ) - quinoxaline bitartrate ( UK-14304 ) were examined using the Halpern pressure myograph .
	manualset3
133610	2	406309	13	NULL	NULL	0	NULL	60 mmHg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Responses of isolated , 60 mmHg ` pressurized ' segments of the distal caudal artery of adult and juvenile Wistar rats to melatonin and the selective alpha 2-adrenoceptor agonist 5-bromo-6 - ( 2-imidazolin-2-ylamino ) - quinoxaline bitartrate ( UK-14304 ) were examined using the Halpern pressure myograph .
	manualset3
133611	3	406309	13	NULL	NULL	0	NULL	segments	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Responses of isolated , 60 mmHg ` pressurized ' segments of the distal caudal artery of adult and juvenile Wistar rats to melatonin and the selective alpha 2-adrenoceptor agonist 5-bromo-6 - ( 2-imidazolin-2-ylamino ) - quinoxaline bitartrate ( UK-14304 ) were examined using the Halpern pressure myograph .
	manualset3
133612	4	406309	13	NULL	NULL	0	NULL	distal caudal artery 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Responses of isolated , 60 mmHg ` pressurized ' segments of the distal caudal artery of adult and juvenile Wistar rats to melatonin and the selective alpha 2-adrenoceptor agonist 5-bromo-6 - ( 2-imidazolin-2-ylamino ) - quinoxaline bitartrate ( UK-14304 ) were examined using the Halpern pressure myograph .
	manualset3
133613	5	406309	13	NULL	NULL	0	NULL	adult Wistar rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Responses of isolated , 60 mmHg ` pressurized ' segments of the distal caudal artery of adult and juvenile Wistar rats to melatonin and the selective alpha 2-adrenoceptor agonist 5-bromo-6 - ( 2-imidazolin-2-ylamino ) - quinoxaline bitartrate ( UK-14304 ) were examined using the Halpern pressure myograph .
	manualset3
133614	6	406309	13	NULL	NULL	0	NULL	juvenile Wistar rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Responses of isolated , 60 mmHg ` pressurized ' segments of the distal caudal artery of adult and juvenile Wistar rats to melatonin and the selective alpha 2-adrenoceptor agonist 5-bromo-6 - ( 2-imidazolin-2-ylamino ) - quinoxaline bitartrate ( UK-14304 ) were examined using the Halpern pressure myograph .
	manualset3
133615	7	406309	13	NULL	NULL	0	NULL	melatonin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Responses of isolated , 60 mmHg ` pressurized ' segments of the distal caudal artery of adult and juvenile Wistar rats to melatonin and the selective alpha 2-adrenoceptor agonist 5-bromo-6 - ( 2-imidazolin-2-ylamino ) - quinoxaline bitartrate ( UK-14304 ) were examined using the Halpern pressure myograph .
	manualset3
133616	8	406309	13	NULL	NULL	0	NULL	selective alpha 2-adrenoceptor agonist 5-bromo-6 - ( 2-imidazolin-2-ylamino ) - quinoxaline bitartrate ( UK-14304 ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Responses of isolated , 60 mmHg ` pressurized ' segments of the distal caudal artery of adult and juvenile Wistar rats to melatonin and the selective alpha 2-adrenoceptor agonist 5-bromo-6 - ( 2-imidazolin-2-ylamino ) - quinoxaline bitartrate ( UK-14304 ) were examined using the Halpern pressure myograph .
	manualset3
133617	9	406309	13	NULL	NULL	0	NULL	Halpern pressure myograph	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Responses of isolated , 60 mmHg ` pressurized ' segments of the distal caudal artery of adult and juvenile Wistar rats to melatonin and the selective alpha 2-adrenoceptor agonist 5-bromo-6 - ( 2-imidazolin-2-ylamino ) - quinoxaline bitartrate ( UK-14304 ) were examined using the Halpern pressure myograph .
	manualset3
133618	1	406310	13	NULL	NULL	0	NULL	Responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Responses to combination chemotherapy have been reported in patients with collecting duct carcinoma and the sarcomatoid variant of renal cancer .
	manualset3
133619	2	406310	13	NULL	NULL	0	NULL	combination chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Responses to combination chemotherapy have been reported in patients with collecting duct carcinoma and the sarcomatoid variant of renal cancer .
	manualset3
133620	3	406310	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Responses to combination chemotherapy have been reported in patients with collecting duct carcinoma and the sarcomatoid variant of renal cancer .
	manualset3
133621	4	406310	13	NULL	NULL	0	NULL	 collecting duct carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Responses to combination chemotherapy have been reported in patients with collecting duct carcinoma and the sarcomatoid variant of renal cancer .
	manualset3
133622	5	406310	13	NULL	NULL	0	NULL	sarcomatoid variant of renal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Responses to combination chemotherapy have been reported in patients with collecting duct carcinoma and the sarcomatoid variant of renal cancer .
	manualset3
133623	1	406311	13	NULL	NULL	0	NULL	Responses 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Responses to the postural change and orthostatic dysregulation symptoms : a population study on Japanese junior and senior high school students .
	manualset3
133624	2	406311	13	NULL	NULL	0	NULL	postural change 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Responses to the postural change and orthostatic dysregulation symptoms : a population study on Japanese junior and senior high school students .
	manualset3
133625	3	406311	13	NULL	NULL	0	NULL	orthostatic dysregulation symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Responses to the postural change and orthostatic dysregulation symptoms : a population study on Japanese junior and senior high school students .
	manualset3
133626	4	406311	13	NULL	NULL	0	NULL	population study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Responses to the postural change and orthostatic dysregulation symptoms : a population study on Japanese junior and senior high school students .
	manualset3
133627	5	406311	13	NULL	NULL	0	NULL	Japanese junior school students 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Responses to the postural change and orthostatic dysregulation symptoms : a population study on Japanese junior and senior high school students .
	manualset3
133628	6	406311	13	NULL	NULL	0	NULL	Japanese senior high school students	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Responses to the postural change and orthostatic dysregulation symptoms : a population study on Japanese junior and senior high school students .
	manualset3
133629	1	406312	13	NULL	NULL	0	NULL	multivariate analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A multivariate analysis was performed , where the dependent variables were : the cumulative length of all hospitalizations , the mean duration of hospitalization and the mean length of stay out of hospital .
	manualset3
133630	2	406312	13	NULL	NULL	0	NULL	variables	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A multivariate analysis was performed , where the dependent variables were : the cumulative length of all hospitalizations , the mean duration of hospitalization and the mean length of stay out of hospital .
	manualset3
133631	3	406312	13	NULL	NULL	0	NULL	cumulative length	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A multivariate analysis was performed , where the dependent variables were : the cumulative length of all hospitalizations , the mean duration of hospitalization and the mean length of stay out of hospital .
	manualset3
133632	4	406312	13	NULL	NULL	0	NULL	hospitalizations 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A multivariate analysis was performed , where the dependent variables were : the cumulative length of all hospitalizations , the mean duration of hospitalization and the mean length of stay out of hospital .
	manualset3
133633	5	406312	13	NULL	NULL	0	NULL	mean duration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A multivariate analysis was performed , where the dependent variables were : the cumulative length of all hospitalizations , the mean duration of hospitalization and the mean length of stay out of hospital .
	manualset3
133634	6	406312	13	NULL	NULL	0	NULL	hospitalization 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A multivariate analysis was performed , where the dependent variables were : the cumulative length of all hospitalizations , the mean duration of hospitalization and the mean length of stay out of hospital .
	manualset3
133635	7	406312	13	NULL	NULL	0	NULL	mean length	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A multivariate analysis was performed , where the dependent variables were : the cumulative length of all hospitalizations , the mean duration of hospitalization and the mean length of stay out of hospital .
	manualset3
133636	8	406312	13	NULL	NULL	0	NULL	stay	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A multivariate analysis was performed , where the dependent variables were : the cumulative length of all hospitalizations , the mean duration of hospitalization and the mean length of stay out of hospital .
	manualset3
133637	9	406312	13	NULL	NULL	0	NULL	hospital	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A multivariate analysis was performed , where the dependent variables were : the cumulative length of all hospitalizations , the mean duration of hospitalization and the mean length of stay out of hospital .
	manualset3
133638	1	406313	13	NULL	NULL	0	NULL	Restaging laparotomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Restaging laparotomy in the management of the non-Hodgkin lymphomas .
	manualset3
133639	2	406313	13	NULL	NULL	0	NULL	management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Restaging laparotomy in the management of the non-Hodgkin lymphomas .
	manualset3
133640	3	406313	13	NULL	NULL	0	NULL	non-Hodgkin lymphomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Restaging laparotomy in the management of the non-Hodgkin lymphomas .
	manualset3
133641	1	406314	13	NULL	NULL	0	NULL	Restaging surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Restaging surgery for women with borderline ovarian tumors : results of a French multicenter study .
	manualset3
133642	2	406314	13	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Restaging surgery for women with borderline ovarian tumors : results of a French multicenter study .
	manualset3
133643	3	406314	13	NULL	NULL	0	NULL	borderline ovarian tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Restaging surgery for women with borderline ovarian tumors : results of a French multicenter study .
	manualset3
133644	4	406314	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Restaging surgery for women with borderline ovarian tumors : results of a French multicenter study .
	manualset3
133645	5	406314	13	NULL	NULL	0	NULL	French multicenter study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Restaging surgery for women with borderline ovarian tumors : results of a French multicenter study .
	manualset3
133646	1	406315	13	NULL	NULL	NULL	NULL	Resting breathing frequency	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Resting breathing frequency is proportional to M-0 .21 , therefore dead space ventilation ( VD ) can be calculated to be proportional to M0 .86 .
	manualset3
133647	2	406315	13	NULL	NULL	0	NULL	M-0 .21	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Resting breathing frequency is proportional to M-0 .21 , therefore dead space ventilation ( VD ) can be calculated to be proportional to M0 .86 .
	manualset3
133648	3	406315	13	NULL	NULL	0	NULL	dead space ventilation ( VD )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Resting breathing frequency is proportional to M-0 .21 , therefore dead space ventilation ( VD ) can be calculated to be proportional to M0 .86 .
	manualset3
133649	4	406315	13	NULL	NULL	0	NULL	M0 .86 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Resting breathing frequency is proportional to M-0 .21 , therefore dead space ventilation ( VD ) can be calculated to be proportional to M0 .86 .
	manualset3
133650	1	406316	13	NULL	NULL	NULL	NULL	Resting oxygen consumption	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Resting oxygen consumption was measured in anaesthetized male and female common marmosets ( Callithrix jacchus ) at 29 degrees C. Injection of noradrenaline caused a marked increase in oxygen consumption ( 63 % ) , but this response was lower in males .
	manualset3
133651	2	406316	13	NULL	NULL	0	NULL	male common marmosets	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Resting oxygen consumption was measured in anaesthetized male and female common marmosets ( Callithrix jacchus ) at 29 degrees C. Injection of noradrenaline caused a marked increase in oxygen consumption ( 63 % ) , but this response was lower in males .
	manualset3
133652	3	406316	13	NULL	NULL	0	NULL	female common marmosets	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Resting oxygen consumption was measured in anaesthetized male and female common marmosets ( Callithrix jacchus ) at 29 degrees C. Injection of noradrenaline caused a marked increase in oxygen consumption ( 63 % ) , but this response was lower in males .
	manualset3
133653	4	406316	13	NULL	NULL	0	NULL	Callithrix jacchus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Resting oxygen consumption was measured in anaesthetized male and female common marmosets ( Callithrix jacchus ) at 29 degrees C. Injection of noradrenaline caused a marked increase in oxygen consumption ( 63 % ) , but this response was lower in males .
	manualset3
133654	5	406316	13	NULL	NULL	0	NULL	29 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Resting oxygen consumption was measured in anaesthetized male and female common marmosets ( Callithrix jacchus ) at 29 degrees C. Injection of noradrenaline caused a marked increase in oxygen consumption ( 63 % ) , but this response was lower in males .
	manualset3
133655	6	406316	13	NULL	NULL	0	NULL	Injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Resting oxygen consumption was measured in anaesthetized male and female common marmosets ( Callithrix jacchus ) at 29 degrees C. Injection of noradrenaline caused a marked increase in oxygen consumption ( 63 % ) , but this response was lower in males .
	manualset3
133656	7	406316	13	NULL	NULL	0	NULL	noradrenaline 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Resting oxygen consumption was measured in anaesthetized male and female common marmosets ( Callithrix jacchus ) at 29 degrees C. Injection of noradrenaline caused a marked increase in oxygen consumption ( 63 % ) , but this response was lower in males .
	manualset3
133657	8	406316	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Resting oxygen consumption was measured in anaesthetized male and female common marmosets ( Callithrix jacchus ) at 29 degrees C. Injection of noradrenaline caused a marked increase in oxygen consumption ( 63 % ) , but this response was lower in males .
	manualset3
133658	9	406316	13	NULL	NULL	NULL	NULL	oxygen consumption	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Resting oxygen consumption was measured in anaesthetized male and female common marmosets ( Callithrix jacchus ) at 29 degrees C. Injection of noradrenaline caused a marked increase in oxygen consumption ( 63 % ) , but this response was lower in males .
	manualset3
133659	10	406316	13	NULL	NULL	0	NULL	63 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Resting oxygen consumption was measured in anaesthetized male and female common marmosets ( Callithrix jacchus ) at 29 degrees C. Injection of noradrenaline caused a marked increase in oxygen consumption ( 63 % ) , but this response was lower in males .
	manualset3
133660	11	406316	13	NULL	NULL	0	NULL	response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Resting oxygen consumption was measured in anaesthetized male and female common marmosets ( Callithrix jacchus ) at 29 degrees C. Injection of noradrenaline caused a marked increase in oxygen consumption ( 63 % ) , but this response was lower in males .
	manualset3
133661	12	406316	13	NULL	NULL	NULL	NULL	males	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Resting oxygen consumption was measured in anaesthetized male and female common marmosets ( Callithrix jacchus ) at 29 degrees C. Injection of noradrenaline caused a marked increase in oxygen consumption ( 63 % ) , but this response was lower in males .
	manualset3
133662	1	406317	13	NULL	NULL	0	NULL	Restoration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Restoration on tissue antioxidants by fenugreek seeds ( Trigonella Foenum Graecum ) in alloxan-diabetic rats .
	manualset3
133663	2	406317	13	NULL	NULL	0	NULL	tissue antioxidants	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Restoration on tissue antioxidants by fenugreek seeds ( Trigonella Foenum Graecum ) in alloxan-diabetic rats .
	manualset3
133664	3	406317	13	NULL	NULL	0	NULL	fenugreek seeds	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Restoration on tissue antioxidants by fenugreek seeds ( Trigonella Foenum Graecum ) in alloxan-diabetic rats .
	manualset3
133665	4	406317	13	NULL	NULL	0	NULL	 Trigonella Foenum Graecum 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Restoration on tissue antioxidants by fenugreek seeds ( Trigonella Foenum Graecum ) in alloxan-diabetic rats .
	manualset3
133666	5	406317	13	NULL	NULL	0	NULL	alloxan-diabetic rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Restoration on tissue antioxidants by fenugreek seeds ( Trigonella Foenum Graecum ) in alloxan-diabetic rats .
	manualset3
133667	1	406318	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Restrained patients were eight times more likely to die during hospitalization ( 24 % v 3 % ; P less than 0.01 ) .
	manualset3
133668	2	406318	13	NULL	NULL	0	NULL	eight times	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Restrained patients were eight times more likely to die during hospitalization ( 24 % v 3 % ; P less than 0.01 ) .
	manualset3
133669	3	406318	13	NULL	NULL	0	NULL	hospitalization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Restrained patients were eight times more likely to die during hospitalization ( 24 % v 3 % ; P less than 0.01 ) .
	manualset3
133670	4	406318	13	NULL	NULL	0	NULL	24 % v 3 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Restrained patients were eight times more likely to die during hospitalization ( 24 % v 3 % ; P less than 0.01 ) .
	manualset3
133671	5	406318	13	NULL	NULL	0	NULL	P less than 0.01 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Restrained patients were eight times more likely to die during hospitalization ( 24 % v 3 % ; P less than 0.01 ) .
	manualset3
133672	1	406319	13	NULL	NULL	0	NULL	colectomy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Restricting colectomy to medical indications during childhood will minimize the complications of colectomy without exposing the patient to risks greater than those of surgery itself .
	manualset3
133673	2	406319	13	NULL	NULL	0	NULL	medical indications 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Restricting colectomy to medical indications during childhood will minimize the complications of colectomy without exposing the patient to risks greater than those of surgery itself .
	manualset3
133674	3	406319	13	NULL	NULL	0	NULL	childhood 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Restricting colectomy to medical indications during childhood will minimize the complications of colectomy without exposing the patient to risks greater than those of surgery itself .
	manualset3
133675	4	406319	13	NULL	NULL	0	NULL	complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Restricting colectomy to medical indications during childhood will minimize the complications of colectomy without exposing the patient to risks greater than those of surgery itself .
	manualset3
133676	5	406319	13	NULL	NULL	0	NULL	colectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Restricting colectomy to medical indications during childhood will minimize the complications of colectomy without exposing the patient to risks greater than those of surgery itself .
	manualset3
133677	6	406319	13	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Restricting colectomy to medical indications during childhood will minimize the complications of colectomy without exposing the patient to risks greater than those of surgery itself .
	manualset3
133678	7	406319	13	NULL	NULL	0	NULL	risks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Restricting colectomy to medical indications during childhood will minimize the complications of colectomy without exposing the patient to risks greater than those of surgery itself .
	manualset3
133679	8	406319	13	NULL	NULL	0	NULL	surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Restricting colectomy to medical indications during childhood will minimize the complications of colectomy without exposing the patient to risks greater than those of surgery itself .
	manualset3
133680	1	406320	13	NULL	NULL	0	NULL	Restriction fragment length polymorphisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Restriction fragment length polymorphisms can be used to distinguish blood and marrow cells from close relatives .
	manualset3
133681	2	406320	13	NULL	NULL	0	NULL	blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Restriction fragment length polymorphisms can be used to distinguish blood and marrow cells from close relatives .
	manualset3
133682	3	406320	13	NULL	NULL	0	NULL	marrow cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Restriction fragment length polymorphisms can be used to distinguish blood and marrow cells from close relatives .
	manualset3
133683	4	406320	13	NULL	NULL	NULL	NULL	relatives 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Restriction fragment length polymorphisms can be used to distinguish blood and marrow cells from close relatives .
	manualset3
133684	1	406321	13	NULL	NULL	0	NULL	 multivariate linear model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A multivariate linear model put in evidence that in males the best collection site in terms of yield is located in the abdomen , whereas in females the biopsy region do not influence cell recovery ; the collection technique , the age , and the body mass index of donor seem not to influence the cell yield .
	manualset3
133685	2	406321	13	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A multivariate linear model put in evidence that in males the best collection site in terms of yield is located in the abdomen , whereas in females the biopsy region do not influence cell recovery ; the collection technique , the age , and the body mass index of donor seem not to influence the cell yield .
	manualset3
133686	3	406321	13	NULL	NULL	0	NULL	males	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A multivariate linear model put in evidence that in males the best collection site in terms of yield is located in the abdomen , whereas in females the biopsy region do not influence cell recovery ; the collection technique , the age , and the body mass index of donor seem not to influence the cell yield .
	manualset3
133687	4	406321	13	NULL	NULL	0	NULL	collection site	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A multivariate linear model put in evidence that in males the best collection site in terms of yield is located in the abdomen , whereas in females the biopsy region do not influence cell recovery ; the collection technique , the age , and the body mass index of donor seem not to influence the cell yield .
	manualset3
133688	5	406321	13	NULL	NULL	0	NULL	terms of yield	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A multivariate linear model put in evidence that in males the best collection site in terms of yield is located in the abdomen , whereas in females the biopsy region do not influence cell recovery ; the collection technique , the age , and the body mass index of donor seem not to influence the cell yield .
	manualset3
133689	6	406321	13	NULL	NULL	0	NULL	abdomen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A multivariate linear model put in evidence that in males the best collection site in terms of yield is located in the abdomen , whereas in females the biopsy region do not influence cell recovery ; the collection technique , the age , and the body mass index of donor seem not to influence the cell yield .
	manualset3
133690	7	406321	13	NULL	NULL	0	NULL	females 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A multivariate linear model put in evidence that in males the best collection site in terms of yield is located in the abdomen , whereas in females the biopsy region do not influence cell recovery ; the collection technique , the age , and the body mass index of donor seem not to influence the cell yield .
	manualset3
133691	8	406321	13	NULL	NULL	0	NULL	biopsy region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A multivariate linear model put in evidence that in males the best collection site in terms of yield is located in the abdomen , whereas in females the biopsy region do not influence cell recovery ; the collection technique , the age , and the body mass index of donor seem not to influence the cell yield .
	manualset3
133692	9	406321	13	NULL	NULL	NULL	NULL	cell recovery	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A multivariate linear model put in evidence that in males the best collection site in terms of yield is located in the abdomen , whereas in females the biopsy region do not influence cell recovery ; the collection technique , the age , and the body mass index of donor seem not to influence the cell yield .
	manualset3
133693	10	406321	13	NULL	NULL	NULL	NULL	collection technique	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A multivariate linear model put in evidence that in males the best collection site in terms of yield is located in the abdomen , whereas in females the biopsy region do not influence cell recovery ; the collection technique , the age , and the body mass index of donor seem not to influence the cell yield .
	manualset3
133694	11	406321	13	NULL	NULL	0	NULL	age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A multivariate linear model put in evidence that in males the best collection site in terms of yield is located in the abdomen , whereas in females the biopsy region do not influence cell recovery ; the collection technique , the age , and the body mass index of donor seem not to influence the cell yield .
	manualset3
133695	12	406321	13	NULL	NULL	0	NULL	body mass index 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A multivariate linear model put in evidence that in males the best collection site in terms of yield is located in the abdomen , whereas in females the biopsy region do not influence cell recovery ; the collection technique , the age , and the body mass index of donor seem not to influence the cell yield .
	manualset3
133696	13	406321	13	NULL	NULL	0	NULL	donor	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A multivariate linear model put in evidence that in males the best collection site in terms of yield is located in the abdomen , whereas in females the biopsy region do not influence cell recovery ; the collection technique , the age , and the body mass index of donor seem not to influence the cell yield .
	manualset3
133697	14	406321	13	NULL	NULL	0	NULL	cell yield 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A multivariate linear model put in evidence that in males the best collection site in terms of yield is located in the abdomen , whereas in females the biopsy region do not influence cell recovery ; the collection technique , the age , and the body mass index of donor seem not to influence the cell yield .
	manualset3
133698	1	406322	13	NULL	NULL	0	NULL	Restriction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Restriction of colposcopy referral to women with definitely abnormal PAPNET readings would have reduced referrals to 31 % , but the sensitivity of the triage would have dropped to 51 % of biopsy-confirmed lesions .
	manualset3
133699	2	406322	13	NULL	NULL	0	NULL	colposcopy referral 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Restriction of colposcopy referral to women with definitely abnormal PAPNET readings would have reduced referrals to 31 % , but the sensitivity of the triage would have dropped to 51 % of biopsy-confirmed lesions .
	manualset3
133700	3	406322	13	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Restriction of colposcopy referral to women with definitely abnormal PAPNET readings would have reduced referrals to 31 % , but the sensitivity of the triage would have dropped to 51 % of biopsy-confirmed lesions .
	manualset3
133701	4	406322	13	NULL	NULL	0	NULL	abnormal PAPNET readings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Restriction of colposcopy referral to women with definitely abnormal PAPNET readings would have reduced referrals to 31 % , but the sensitivity of the triage would have dropped to 51 % of biopsy-confirmed lesions .
	manualset3
133702	5	406322	13	NULL	NULL	0	NULL	referrals	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Restriction of colposcopy referral to women with definitely abnormal PAPNET readings would have reduced referrals to 31 % , but the sensitivity of the triage would have dropped to 51 % of biopsy-confirmed lesions .
	manualset3
133703	6	406322	13	NULL	NULL	0	NULL	31 %  	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Restriction of colposcopy referral to women with definitely abnormal PAPNET readings would have reduced referrals to 31 % , but the sensitivity of the triage would have dropped to 51 % of biopsy-confirmed lesions .
	manualset3
133704	7	406322	13	NULL	NULL	0	NULL	sensitivity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Restriction of colposcopy referral to women with definitely abnormal PAPNET readings would have reduced referrals to 31 % , but the sensitivity of the triage would have dropped to 51 % of biopsy-confirmed lesions .
	manualset3
133705	8	406322	13	NULL	NULL	0	NULL	triage	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Restriction of colposcopy referral to women with definitely abnormal PAPNET readings would have reduced referrals to 31 % , but the sensitivity of the triage would have dropped to 51 % of biopsy-confirmed lesions .
	manualset3
133706	9	406322	13	NULL	NULL	0	NULL	51 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Restriction of colposcopy referral to women with definitely abnormal PAPNET readings would have reduced referrals to 31 % , but the sensitivity of the triage would have dropped to 51 % of biopsy-confirmed lesions .
	manualset3
133707	10	406322	13	NULL	NULL	0	NULL	biopsy-confirmed lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Restriction of colposcopy referral to women with definitely abnormal PAPNET readings would have reduced referrals to 31 % , but the sensitivity of the triage would have dropped to 51 % of biopsy-confirmed lesions .
	manualset3
133708	1	406323	13	NULL	NULL	0	NULL	Restriction site mapping	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Restriction site mapping of the homologous cloned BamHI `` H '' fragment from the nontransforming EBV ( P3HR-1 ) isolate revealed that a contiguous 6 , 650-bp region including the entire NotI repeat cluster has been deleted from the BamHI-H , - Y , and - W regions of the P3HR-1 genome .
	manualset3
133709	2	406323	13	NULL	NULL	0	NULL	homologous cloned BamHI `` H '' fragment	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Restriction site mapping of the homologous cloned BamHI `` H '' fragment from the nontransforming EBV ( P3HR-1 ) isolate revealed that a contiguous 6 , 650-bp region including the entire NotI repeat cluster has been deleted from the BamHI-H , - Y , and - W regions of the P3HR-1 genome .
	manualset3
133710	3	406323	13	NULL	NULL	0	NULL	nontransforming EBV ( P3HR-1 ) isolate	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Restriction site mapping of the homologous cloned BamHI `` H '' fragment from the nontransforming EBV ( P3HR-1 ) isolate revealed that a contiguous 6 , 650-bp region including the entire NotI repeat cluster has been deleted from the BamHI-H , - Y , and - W regions of the P3HR-1 genome .
	manualset3
133711	4	406323	13	NULL	NULL	0	NULL	contiguous 6 , 650-bp region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Restriction site mapping of the homologous cloned BamHI `` H '' fragment from the nontransforming EBV ( P3HR-1 ) isolate revealed that a contiguous 6 , 650-bp region including the entire NotI repeat cluster has been deleted from the BamHI-H , - Y , and - W regions of the P3HR-1 genome .
	manualset3
133712	5	406323	13	NULL	NULL	0	NULL	NotI repeat cluster 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Restriction site mapping of the homologous cloned BamHI `` H '' fragment from the nontransforming EBV ( P3HR-1 ) isolate revealed that a contiguous 6 , 650-bp region including the entire NotI repeat cluster has been deleted from the BamHI-H , - Y , and - W regions of the P3HR-1 genome .
	manualset3
133713	6	406323	13	NULL	NULL	0	NULL	BamHI-H regions	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Restriction site mapping of the homologous cloned BamHI `` H '' fragment from the nontransforming EBV ( P3HR-1 ) isolate revealed that a contiguous 6 , 650-bp region including the entire NotI repeat cluster has been deleted from the BamHI-H , - Y , and - W regions of the P3HR-1 genome .
	manualset3
133714	7	406323	13	NULL	NULL	0	NULL	BamHI-Y regions	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Restriction site mapping of the homologous cloned BamHI `` H '' fragment from the nontransforming EBV ( P3HR-1 ) isolate revealed that a contiguous 6 , 650-bp region including the entire NotI repeat cluster has been deleted from the BamHI-H , - Y , and - W regions of the P3HR-1 genome .
	manualset3
133715	8	406323	13	NULL	NULL	0	NULL	BamHI-W regions	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Restriction site mapping of the homologous cloned BamHI `` H '' fragment from the nontransforming EBV ( P3HR-1 ) isolate revealed that a contiguous 6 , 650-bp region including the entire NotI repeat cluster has been deleted from the BamHI-H , - Y , and - W regions of the P3HR-1 genome .
	manualset3
133716	9	406323	13	NULL	NULL	0	NULL	P3HR-1 genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Restriction site mapping of the homologous cloned BamHI `` H '' fragment from the nontransforming EBV ( P3HR-1 ) isolate revealed that a contiguous 6 , 650-bp region including the entire NotI repeat cluster has been deleted from the BamHI-H , - Y , and - W regions of the P3HR-1 genome .
	manualset3
133717	1	406324	13	NULL	NULL	0	NULL	formation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Resultant formation of abnormal film matrices could initiate pathological transformations in the morphology , metabolism , and replication of the affected cells .
	manualset3
133718	2	406324	13	NULL	NULL	0	NULL	abnormal film matrices 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Resultant formation of abnormal film matrices could initiate pathological transformations in the morphology , metabolism , and replication of the affected cells .
	manualset3
133719	3	406324	13	NULL	NULL	0	NULL	pathological transformations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Resultant formation of abnormal film matrices could initiate pathological transformations in the morphology , metabolism , and replication of the affected cells .
	manualset3
133720	4	406324	13	NULL	NULL	0	NULL	morphology 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Resultant formation of abnormal film matrices could initiate pathological transformations in the morphology , metabolism , and replication of the affected cells .
	manualset3
133721	5	406324	13	NULL	NULL	0	NULL	metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Resultant formation of abnormal film matrices could initiate pathological transformations in the morphology , metabolism , and replication of the affected cells .
	manualset3
133722	6	406324	13	NULL	NULL	0	NULL	replication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Resultant formation of abnormal film matrices could initiate pathological transformations in the morphology , metabolism , and replication of the affected cells .
	manualset3
133723	7	406324	13	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Resultant formation of abnormal film matrices could initiate pathological transformations in the morphology , metabolism , and replication of the affected cells .
	manualset3
133724	1	406325	13	NULL	NULL	0	NULL	hypertensive systemic mean arterial BPs 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Resulting hypertensive systemic mean arterial BPs were 99 + / - 8 mm Hg in the 15 control pups and 93 + / - 15 mm Hg in the 15 phenobarbital sodium-treated pups ( not statistically significantly different ) .
	manualset3
133725	2	406325	13	NULL	NULL	0	NULL	99 + / - 8 mm Hg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Resulting hypertensive systemic mean arterial BPs were 99 + / - 8 mm Hg in the 15 control pups and 93 + / - 15 mm Hg in the 15 phenobarbital sodium-treated pups ( not statistically significantly different ) .
	manualset3
133726	3	406325	13	NULL	NULL	0	NULL	15 control pups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Resulting hypertensive systemic mean arterial BPs were 99 + / - 8 mm Hg in the 15 control pups and 93 + / - 15 mm Hg in the 15 phenobarbital sodium-treated pups ( not statistically significantly different ) .
	manualset3
133727	4	406325	13	NULL	NULL	0	NULL	93 + / - 15 mm Hg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Resulting hypertensive systemic mean arterial BPs were 99 + / - 8 mm Hg in the 15 control pups and 93 + / - 15 mm Hg in the 15 phenobarbital sodium-treated pups ( not statistically significantly different ) .
	manualset3
133728	5	406325	13	NULL	NULL	0	NULL	15 phenobarbital sodium-treated pups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Resulting hypertensive systemic mean arterial BPs were 99 + / - 8 mm Hg in the 15 control pups and 93 + / - 15 mm Hg in the 15 phenobarbital sodium-treated pups ( not statistically significantly different ) .
	manualset3
133772	1	406326	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Our checklist includes questions about the risk to research participants , sponsorship of the study , control of data analysis , freedom to publish results , the impact of the research on industry customers , openness to input from all partners , sharing results before publication , and publication of industry-specific data .
	manualset3
133774	2	406326	13	NULL	NULL	0	NULL	checklist 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Our checklist includes questions about the risk to research participants , sponsorship of the study , control of data analysis , freedom to publish results , the impact of the research on industry customers , openness to input from all partners , sharing results before publication , and publication of industry-specific data .
	manualset3
133775	3	406326	13	NULL	NULL	0	NULL	questions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Our checklist includes questions about the risk to research participants , sponsorship of the study , control of data analysis , freedom to publish results , the impact of the research on industry customers , openness to input from all partners , sharing results before publication , and publication of industry-specific data .
	manualset3
133777	4	406326	13	NULL	NULL	0	NULL	risk 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Our checklist includes questions about the risk to research participants , sponsorship of the study , control of data analysis , freedom to publish results , the impact of the research on industry customers , openness to input from all partners , sharing results before publication , and publication of industry-specific data .
	manualset3
133779	5	406326	13	NULL	NULL	0	NULL	research participants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Our checklist includes questions about the risk to research participants , sponsorship of the study , control of data analysis , freedom to publish results , the impact of the research on industry customers , openness to input from all partners , sharing results before publication , and publication of industry-specific data .
	manualset3
133781	6	406326	13	NULL	NULL	0	NULL	sponsorship	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Our checklist includes questions about the risk to research participants , sponsorship of the study , control of data analysis , freedom to publish results , the impact of the research on industry customers , openness to input from all partners , sharing results before publication , and publication of industry-specific data .
	manualset3
133783	7	406326	13	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Our checklist includes questions about the risk to research participants , sponsorship of the study , control of data analysis , freedom to publish results , the impact of the research on industry customers , openness to input from all partners , sharing results before publication , and publication of industry-specific data .
	manualset3
133785	8	406326	13	NULL	NULL	0	NULL	control 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Our checklist includes questions about the risk to research participants , sponsorship of the study , control of data analysis , freedom to publish results , the impact of the research on industry customers , openness to input from all partners , sharing results before publication , and publication of industry-specific data .
	manualset3
133898	9	406326	13	NULL	NULL	0	NULL	data analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Our checklist includes questions about the risk to research participants , sponsorship of the study , control of data analysis , freedom to publish results , the impact of the research on industry customers , openness to input from all partners , sharing results before publication , and publication of industry-specific data .
	manualset3
133899	10	406326	13	NULL	NULL	0	NULL	freedom	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Our checklist includes questions about the risk to research participants , sponsorship of the study , control of data analysis , freedom to publish results , the impact of the research on industry customers , openness to input from all partners , sharing results before publication , and publication of industry-specific data .
	manualset3
133900	11	406326	13	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Our checklist includes questions about the risk to research participants , sponsorship of the study , control of data analysis , freedom to publish results , the impact of the research on industry customers , openness to input from all partners , sharing results before publication , and publication of industry-specific data .
	manualset3
133901	12	406326	13	NULL	NULL	0	NULL	impact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Our checklist includes questions about the risk to research participants , sponsorship of the study , control of data analysis , freedom to publish results , the impact of the research on industry customers , openness to input from all partners , sharing results before publication , and publication of industry-specific data .
	manualset3
133902	13	406326	13	NULL	NULL	0	NULL	research 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Our checklist includes questions about the risk to research participants , sponsorship of the study , control of data analysis , freedom to publish results , the impact of the research on industry customers , openness to input from all partners , sharing results before publication , and publication of industry-specific data .
	manualset3
133903	14	406326	13	NULL	NULL	0	NULL	industry customers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Our checklist includes questions about the risk to research participants , sponsorship of the study , control of data analysis , freedom to publish results , the impact of the research on industry customers , openness to input from all partners , sharing results before publication , and publication of industry-specific data .
	manualset3
133904	15	406326	13	NULL	NULL	0	NULL	openness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Our checklist includes questions about the risk to research participants , sponsorship of the study , control of data analysis , freedom to publish results , the impact of the research on industry customers , openness to input from all partners , sharing results before publication , and publication of industry-specific data .
	manualset3
133905	16	406326	13	NULL	NULL	0	NULL	partners 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Our checklist includes questions about the risk to research participants , sponsorship of the study , control of data analysis , freedom to publish results , the impact of the research on industry customers , openness to input from all partners , sharing results before publication , and publication of industry-specific data .
	manualset3
133906	17	406326	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Our checklist includes questions about the risk to research participants , sponsorship of the study , control of data analysis , freedom to publish results , the impact of the research on industry customers , openness to input from all partners , sharing results before publication , and publication of industry-specific data .
	manualset3
133907	18	406326	13	NULL	NULL	0	NULL	publication	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Our checklist includes questions about the risk to research participants , sponsorship of the study , control of data analysis , freedom to publish results , the impact of the research on industry customers , openness to input from all partners , sharing results before publication , and publication of industry-specific data .
	manualset3
133908	19	406326	13	NULL	NULL	0	NULL	publication 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Our checklist includes questions about the risk to research participants , sponsorship of the study , control of data analysis , freedom to publish results , the impact of the research on industry customers , openness to input from all partners , sharing results before publication , and publication of industry-specific data .
	manualset3
133909	20	406326	13	NULL	NULL	0	NULL	industry-specific data 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Our checklist includes questions about the risk to research participants , sponsorship of the study , control of data analysis , freedom to publish results , the impact of the research on industry customers , openness to input from all partners , sharing results before publication , and publication of industry-specific data .
	manualset3
133758	1	406327	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : A septic insult resulted in significant alterations on hemavet values , free T3 , free T4 and cortisol levels , peritoneal bacteria content and intestinal lung and liver tissue samples of the CLP group .
	manualset3
133759	2	406327	13	NULL	NULL	0	NULL	septic insult	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : A septic insult resulted in significant alterations on hemavet values , free T3 , free T4 and cortisol levels , peritoneal bacteria content and intestinal lung and liver tissue samples of the CLP group .
	manualset3
133760	3	406327	13	NULL	NULL	0	NULL	alterations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : A septic insult resulted in significant alterations on hemavet values , free T3 , free T4 and cortisol levels , peritoneal bacteria content and intestinal lung and liver tissue samples of the CLP group .
	manualset3
133761	4	406327	13	NULL	NULL	0	NULL	hemavet values	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : A septic insult resulted in significant alterations on hemavet values , free T3 , free T4 and cortisol levels , peritoneal bacteria content and intestinal lung and liver tissue samples of the CLP group .
	manualset3
133762	5	406327	13	NULL	NULL	0	NULL	free T3 levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : A septic insult resulted in significant alterations on hemavet values , free T3 , free T4 and cortisol levels , peritoneal bacteria content and intestinal lung and liver tissue samples of the CLP group .
	manualset3
133763	6	406327	13	NULL	NULL	0	NULL	free T4 levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : A septic insult resulted in significant alterations on hemavet values , free T3 , free T4 and cortisol levels , peritoneal bacteria content and intestinal lung and liver tissue samples of the CLP group .
	manualset3
133764	7	406327	13	NULL	NULL	0	NULL	cortisol levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : A septic insult resulted in significant alterations on hemavet values , free T3 , free T4 and cortisol levels , peritoneal bacteria content and intestinal lung and liver tissue samples of the CLP group .
	manualset3
133765	8	406327	13	NULL	NULL	0	NULL	peritoneal bacteria content	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : A septic insult resulted in significant alterations on hemavet values , free T3 , free T4 and cortisol levels , peritoneal bacteria content and intestinal lung and liver tissue samples of the CLP group .
	manualset3
133766	9	406327	13	NULL	NULL	0	NULL	intestinal lung tissue samples	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : A septic insult resulted in significant alterations on hemavet values , free T3 , free T4 and cortisol levels , peritoneal bacteria content and intestinal lung and liver tissue samples of the CLP group .
	manualset3
133767	10	406327	13	NULL	NULL	0	NULL	liver tissue samples	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : A septic insult resulted in significant alterations on hemavet values , free T3 , free T4 and cortisol levels , peritoneal bacteria content and intestinal lung and liver tissue samples of the CLP group .
	manualset3
133769	11	406327	13	NULL	NULL	0	NULL	CLP group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : A septic insult resulted in significant alterations on hemavet values , free T3 , free T4 and cortisol levels , peritoneal bacteria content and intestinal lung and liver tissue samples of the CLP group .
	manualset3
133754	1	406328	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : A significant decrease was found in the values of STS duration .
	manualset3
133755	2	406328	13	NULL	NULL	0	NULL	decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : A significant decrease was found in the values of STS duration .
	manualset3
133756	3	406328	13	NULL	NULL	0	NULL	values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : A significant decrease was found in the values of STS duration .
	manualset3
133757	4	406328	13	NULL	NULL	0	NULL	STS duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : A significant decrease was found in the values of STS duration .
	manualset3
133748	1	406329	13	NULL	NULL	0	NULL	muscle biopsy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A muscle biopsy was taken at rest from m. gastrocnemius of the soccer players and runners , and from m. vastus lateralis of the cyclists .
	manualset3
133749	2	406329	13	NULL	NULL	0	NULL	m. gastrocnemius	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A muscle biopsy was taken at rest from m. gastrocnemius of the soccer players and runners , and from m. vastus lateralis of the cyclists .
	manualset3
133750	3	406329	13	NULL	NULL	0	NULL	soccer players	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A muscle biopsy was taken at rest from m. gastrocnemius of the soccer players and runners , and from m. vastus lateralis of the cyclists .
	manualset3
133751	4	406329	13	NULL	NULL	0	NULL	runners	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A muscle biopsy was taken at rest from m. gastrocnemius of the soccer players and runners , and from m. vastus lateralis of the cyclists .
	manualset3
133752	5	406329	13	NULL	NULL	0	NULL	m. vastus lateralis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A muscle biopsy was taken at rest from m. gastrocnemius of the soccer players and runners , and from m. vastus lateralis of the cyclists .
	manualset3
133753	6	406329	13	NULL	NULL	0	NULL	cyclists 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A muscle biopsy was taken at rest from m. gastrocnemius of the soccer players and runners , and from m. vastus lateralis of the cyclists .
	manualset3
133729	1	406330	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Body mass index ( 48.9 vs. 25.4 kg/m ( 2 ) ) , weight ( 128.6 vs. 71.9 kg ) , serum leptin ( 74.6 vs. 25.2 ng/ml ) , PTH ( 44.5 vs. 28.8 pg/ml ) , fibroblast growth factor 23 ( FGF23 ) ( 42.4 vs. 25.9 pg/ml ) , and bone alkaline phosphatase ( BAP ) ( 25.8 vs. 17.5 U/liter ) were higher , but height ( 162.3 vs. 167.7 cm ) and 1 , 25-dihydroxyvitamin D ( 1 , 25 D ) ( 39.2 vs. 48.7 pg/ml ) were lower in bariatric surgery patients than controls .
	manualset3
133730	2	406330	13	NULL	NULL	0	NULL	Body mass index 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Body mass index ( 48.9 vs. 25.4 kg/m ( 2 ) ) , weight ( 128.6 vs. 71.9 kg ) , serum leptin ( 74.6 vs. 25.2 ng/ml ) , PTH ( 44.5 vs. 28.8 pg/ml ) , fibroblast growth factor 23 ( FGF23 ) ( 42.4 vs. 25.9 pg/ml ) , and bone alkaline phosphatase ( BAP ) ( 25.8 vs. 17.5 U/liter ) were higher , but height ( 162.3 vs. 167.7 cm ) and 1 , 25-dihydroxyvitamin D ( 1 , 25 D ) ( 39.2 vs. 48.7 pg/ml ) were lower in bariatric surgery patients than controls .
	manualset3
133731	3	406330	13	NULL	NULL	0	NULL	48.9 vs. 25.4 kg/m ( 2 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Body mass index ( 48.9 vs. 25.4 kg/m ( 2 ) ) , weight ( 128.6 vs. 71.9 kg ) , serum leptin ( 74.6 vs. 25.2 ng/ml ) , PTH ( 44.5 vs. 28.8 pg/ml ) , fibroblast growth factor 23 ( FGF23 ) ( 42.4 vs. 25.9 pg/ml ) , and bone alkaline phosphatase ( BAP ) ( 25.8 vs. 17.5 U/liter ) were higher , but height ( 162.3 vs. 167.7 cm ) and 1 , 25-dihydroxyvitamin D ( 1 , 25 D ) ( 39.2 vs. 48.7 pg/ml ) were lower in bariatric surgery patients than controls .
	manualset3
133732	4	406330	13	NULL	NULL	0	NULL	weight	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Body mass index ( 48.9 vs. 25.4 kg/m ( 2 ) ) , weight ( 128.6 vs. 71.9 kg ) , serum leptin ( 74.6 vs. 25.2 ng/ml ) , PTH ( 44.5 vs. 28.8 pg/ml ) , fibroblast growth factor 23 ( FGF23 ) ( 42.4 vs. 25.9 pg/ml ) , and bone alkaline phosphatase ( BAP ) ( 25.8 vs. 17.5 U/liter ) were higher , but height ( 162.3 vs. 167.7 cm ) and 1 , 25-dihydroxyvitamin D ( 1 , 25 D ) ( 39.2 vs. 48.7 pg/ml ) were lower in bariatric surgery patients than controls .
	manualset3
133733	5	406330	13	NULL	NULL	0	NULL	128.6 vs. 71.9 kg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Body mass index ( 48.9 vs. 25.4 kg/m ( 2 ) ) , weight ( 128.6 vs. 71.9 kg ) , serum leptin ( 74.6 vs. 25.2 ng/ml ) , PTH ( 44.5 vs. 28.8 pg/ml ) , fibroblast growth factor 23 ( FGF23 ) ( 42.4 vs. 25.9 pg/ml ) , and bone alkaline phosphatase ( BAP ) ( 25.8 vs. 17.5 U/liter ) were higher , but height ( 162.3 vs. 167.7 cm ) and 1 , 25-dihydroxyvitamin D ( 1 , 25 D ) ( 39.2 vs. 48.7 pg/ml ) were lower in bariatric surgery patients than controls .
	manualset3
133734	6	406330	13	NULL	NULL	NULL	NULL	serum leptin 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Results : Body mass index ( 48.9 vs. 25.4 kg/m ( 2 ) ) , weight ( 128.6 vs. 71.9 kg ) , serum leptin ( 74.6 vs. 25.2 ng/ml ) , PTH ( 44.5 vs. 28.8 pg/ml ) , fibroblast growth factor 23 ( FGF23 ) ( 42.4 vs. 25.9 pg/ml ) , and bone alkaline phosphatase ( BAP ) ( 25.8 vs. 17.5 U/liter ) were higher , but height ( 162.3 vs. 167.7 cm ) and 1 , 25-dihydroxyvitamin D ( 1 , 25 D ) ( 39.2 vs. 48.7 pg/ml ) were lower in bariatric surgery patients than controls .
	manualset3
133735	7	406330	13	NULL	NULL	0	NULL	74.6 vs. 25.2 ng/ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Body mass index ( 48.9 vs. 25.4 kg/m ( 2 ) ) , weight ( 128.6 vs. 71.9 kg ) , serum leptin ( 74.6 vs. 25.2 ng/ml ) , PTH ( 44.5 vs. 28.8 pg/ml ) , fibroblast growth factor 23 ( FGF23 ) ( 42.4 vs. 25.9 pg/ml ) , and bone alkaline phosphatase ( BAP ) ( 25.8 vs. 17.5 U/liter ) were higher , but height ( 162.3 vs. 167.7 cm ) and 1 , 25-dihydroxyvitamin D ( 1 , 25 D ) ( 39.2 vs. 48.7 pg/ml ) were lower in bariatric surgery patients than controls .
	manualset3
133736	8	406330	13	NULL	NULL	0	NULL	PTH 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Body mass index ( 48.9 vs. 25.4 kg/m ( 2 ) ) , weight ( 128.6 vs. 71.9 kg ) , serum leptin ( 74.6 vs. 25.2 ng/ml ) , PTH ( 44.5 vs. 28.8 pg/ml ) , fibroblast growth factor 23 ( FGF23 ) ( 42.4 vs. 25.9 pg/ml ) , and bone alkaline phosphatase ( BAP ) ( 25.8 vs. 17.5 U/liter ) were higher , but height ( 162.3 vs. 167.7 cm ) and 1 , 25-dihydroxyvitamin D ( 1 , 25 D ) ( 39.2 vs. 48.7 pg/ml ) were lower in bariatric surgery patients than controls .
	manualset3
133737	9	406330	13	NULL	NULL	0	NULL	44.5 vs. 28.8 pg/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Body mass index ( 48.9 vs. 25.4 kg/m ( 2 ) ) , weight ( 128.6 vs. 71.9 kg ) , serum leptin ( 74.6 vs. 25.2 ng/ml ) , PTH ( 44.5 vs. 28.8 pg/ml ) , fibroblast growth factor 23 ( FGF23 ) ( 42.4 vs. 25.9 pg/ml ) , and bone alkaline phosphatase ( BAP ) ( 25.8 vs. 17.5 U/liter ) were higher , but height ( 162.3 vs. 167.7 cm ) and 1 , 25-dihydroxyvitamin D ( 1 , 25 D ) ( 39.2 vs. 48.7 pg/ml ) were lower in bariatric surgery patients than controls .
	manualset3
133738	10	406330	13	NULL	NULL	0	NULL	fibroblast growth factor 23 ( FGF23 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Body mass index ( 48.9 vs. 25.4 kg/m ( 2 ) ) , weight ( 128.6 vs. 71.9 kg ) , serum leptin ( 74.6 vs. 25.2 ng/ml ) , PTH ( 44.5 vs. 28.8 pg/ml ) , fibroblast growth factor 23 ( FGF23 ) ( 42.4 vs. 25.9 pg/ml ) , and bone alkaline phosphatase ( BAP ) ( 25.8 vs. 17.5 U/liter ) were higher , but height ( 162.3 vs. 167.7 cm ) and 1 , 25-dihydroxyvitamin D ( 1 , 25 D ) ( 39.2 vs. 48.7 pg/ml ) were lower in bariatric surgery patients than controls .
	manualset3
133739	11	406330	13	NULL	NULL	0	NULL	42.4 vs. 25.9 pg/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Body mass index ( 48.9 vs. 25.4 kg/m ( 2 ) ) , weight ( 128.6 vs. 71.9 kg ) , serum leptin ( 74.6 vs. 25.2 ng/ml ) , PTH ( 44.5 vs. 28.8 pg/ml ) , fibroblast growth factor 23 ( FGF23 ) ( 42.4 vs. 25.9 pg/ml ) , and bone alkaline phosphatase ( BAP ) ( 25.8 vs. 17.5 U/liter ) were higher , but height ( 162.3 vs. 167.7 cm ) and 1 , 25-dihydroxyvitamin D ( 1 , 25 D ) ( 39.2 vs. 48.7 pg/ml ) were lower in bariatric surgery patients than controls .
	manualset3
133740	12	406330	13	NULL	NULL	0	NULL	bone alkaline phosphatase ( BAP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Body mass index ( 48.9 vs. 25.4 kg/m ( 2 ) ) , weight ( 128.6 vs. 71.9 kg ) , serum leptin ( 74.6 vs. 25.2 ng/ml ) , PTH ( 44.5 vs. 28.8 pg/ml ) , fibroblast growth factor 23 ( FGF23 ) ( 42.4 vs. 25.9 pg/ml ) , and bone alkaline phosphatase ( BAP ) ( 25.8 vs. 17.5 U/liter ) were higher , but height ( 162.3 vs. 167.7 cm ) and 1 , 25-dihydroxyvitamin D ( 1 , 25 D ) ( 39.2 vs. 48.7 pg/ml ) were lower in bariatric surgery patients than controls .
	manualset3
133741	13	406330	13	NULL	NULL	0	NULL	25.8 vs. 17.5 U/liter	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Body mass index ( 48.9 vs. 25.4 kg/m ( 2 ) ) , weight ( 128.6 vs. 71.9 kg ) , serum leptin ( 74.6 vs. 25.2 ng/ml ) , PTH ( 44.5 vs. 28.8 pg/ml ) , fibroblast growth factor 23 ( FGF23 ) ( 42.4 vs. 25.9 pg/ml ) , and bone alkaline phosphatase ( BAP ) ( 25.8 vs. 17.5 U/liter ) were higher , but height ( 162.3 vs. 167.7 cm ) and 1 , 25-dihydroxyvitamin D ( 1 , 25 D ) ( 39.2 vs. 48.7 pg/ml ) were lower in bariatric surgery patients than controls .
	manualset3
133742	14	406330	13	NULL	NULL	0	NULL	height	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Body mass index ( 48.9 vs. 25.4 kg/m ( 2 ) ) , weight ( 128.6 vs. 71.9 kg ) , serum leptin ( 74.6 vs. 25.2 ng/ml ) , PTH ( 44.5 vs. 28.8 pg/ml ) , fibroblast growth factor 23 ( FGF23 ) ( 42.4 vs. 25.9 pg/ml ) , and bone alkaline phosphatase ( BAP ) ( 25.8 vs. 17.5 U/liter ) were higher , but height ( 162.3 vs. 167.7 cm ) and 1 , 25-dihydroxyvitamin D ( 1 , 25 D ) ( 39.2 vs. 48.7 pg/ml ) were lower in bariatric surgery patients than controls .
	manualset3
133743	15	406330	13	NULL	NULL	0	NULL	162.3 vs. 167.7 cm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Body mass index ( 48.9 vs. 25.4 kg/m ( 2 ) ) , weight ( 128.6 vs. 71.9 kg ) , serum leptin ( 74.6 vs. 25.2 ng/ml ) , PTH ( 44.5 vs. 28.8 pg/ml ) , fibroblast growth factor 23 ( FGF23 ) ( 42.4 vs. 25.9 pg/ml ) , and bone alkaline phosphatase ( BAP ) ( 25.8 vs. 17.5 U/liter ) were higher , but height ( 162.3 vs. 167.7 cm ) and 1 , 25-dihydroxyvitamin D ( 1 , 25 D ) ( 39.2 vs. 48.7 pg/ml ) were lower in bariatric surgery patients than controls .
	manualset3
133744	16	406330	13	NULL	NULL	0	NULL	1 , 25-dihydroxyvitamin D ( 1 , 25 D )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Body mass index ( 48.9 vs. 25.4 kg/m ( 2 ) ) , weight ( 128.6 vs. 71.9 kg ) , serum leptin ( 74.6 vs. 25.2 ng/ml ) , PTH ( 44.5 vs. 28.8 pg/ml ) , fibroblast growth factor 23 ( FGF23 ) ( 42.4 vs. 25.9 pg/ml ) , and bone alkaline phosphatase ( BAP ) ( 25.8 vs. 17.5 U/liter ) were higher , but height ( 162.3 vs. 167.7 cm ) and 1 , 25-dihydroxyvitamin D ( 1 , 25 D ) ( 39.2 vs. 48.7 pg/ml ) were lower in bariatric surgery patients than controls .
	manualset3
133745	17	406330	13	NULL	NULL	0	NULL	39.2 vs. 48.7 pg/ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Body mass index ( 48.9 vs. 25.4 kg/m ( 2 ) ) , weight ( 128.6 vs. 71.9 kg ) , serum leptin ( 74.6 vs. 25.2 ng/ml ) , PTH ( 44.5 vs. 28.8 pg/ml ) , fibroblast growth factor 23 ( FGF23 ) ( 42.4 vs. 25.9 pg/ml ) , and bone alkaline phosphatase ( BAP ) ( 25.8 vs. 17.5 U/liter ) were higher , but height ( 162.3 vs. 167.7 cm ) and 1 , 25-dihydroxyvitamin D ( 1 , 25 D ) ( 39.2 vs. 48.7 pg/ml ) were lower in bariatric surgery patients than controls .
	manualset3
133746	18	406330	13	NULL	NULL	0	NULL	bariatric surgery patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Body mass index ( 48.9 vs. 25.4 kg/m ( 2 ) ) , weight ( 128.6 vs. 71.9 kg ) , serum leptin ( 74.6 vs. 25.2 ng/ml ) , PTH ( 44.5 vs. 28.8 pg/ml ) , fibroblast growth factor 23 ( FGF23 ) ( 42.4 vs. 25.9 pg/ml ) , and bone alkaline phosphatase ( BAP ) ( 25.8 vs. 17.5 U/liter ) were higher , but height ( 162.3 vs. 167.7 cm ) and 1 , 25-dihydroxyvitamin D ( 1 , 25 D ) ( 39.2 vs. 48.7 pg/ml ) were lower in bariatric surgery patients than controls .
	manualset3
133747	19	406330	13	NULL	NULL	0	NULL	controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Body mass index ( 48.9 vs. 25.4 kg/m ( 2 ) ) , weight ( 128.6 vs. 71.9 kg ) , serum leptin ( 74.6 vs. 25.2 ng/ml ) , PTH ( 44.5 vs. 28.8 pg/ml ) , fibroblast growth factor 23 ( FGF23 ) ( 42.4 vs. 25.9 pg/ml ) , and bone alkaline phosphatase ( BAP ) ( 25.8 vs. 17.5 U/liter ) were higher , but height ( 162.3 vs. 167.7 cm ) and 1 , 25-dihydroxyvitamin D ( 1 , 25 D ) ( 39.2 vs. 48.7 pg/ml ) were lower in bariatric surgery patients than controls .
	manualset3
133910	1	406331	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Despite relatively severe cognitive deficits patients were able to carry out a demanding training program with positive results .
	manualset3
133911	2	406331	13	NULL	NULL	0	NULL	severe cognitive deficits patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Despite relatively severe cognitive deficits patients were able to carry out a demanding training program with positive results .
	manualset3
133913	4	406331	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Despite relatively severe cognitive deficits patients were able to carry out a demanding training program with positive results .
	manualset3
133912	1	406332	13	NULL	NULL	NULL	NULL	Results	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Results : Intranasal inoculation of D. farinae-sensitized pDCs significantly inhibited the development of allergic airway inflammation and both Th1 and Th2 immunity .
	manualset3
133914	2	406332	13	NULL	NULL	0	NULL	Intranasal inoculation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Intranasal inoculation of D. farinae-sensitized pDCs significantly inhibited the development of allergic airway inflammation and both Th1 and Th2 immunity .
	manualset3
133915	3	406332	13	NULL	NULL	0	NULL	D. farinae-sensitized pDCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Intranasal inoculation of D. farinae-sensitized pDCs significantly inhibited the development of allergic airway inflammation and both Th1 and Th2 immunity .
	manualset3
133916	4	406332	13	NULL	NULL	0	NULL	development	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Intranasal inoculation of D. farinae-sensitized pDCs significantly inhibited the development of allergic airway inflammation and both Th1 and Th2 immunity .
	manualset3
133917	5	406332	13	NULL	NULL	0	NULL	allergic airway inflammation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Intranasal inoculation of D. farinae-sensitized pDCs significantly inhibited the development of allergic airway inflammation and both Th1 and Th2 immunity .
	manualset3
133918	6	406332	13	NULL	NULL	0	NULL	Th1 immunity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Intranasal inoculation of D. farinae-sensitized pDCs significantly inhibited the development of allergic airway inflammation and both Th1 and Th2 immunity .
	manualset3
133919	7	406332	13	NULL	NULL	0	NULL	Th2 immunity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Intranasal inoculation of D. farinae-sensitized pDCs significantly inhibited the development of allergic airway inflammation and both Th1 and Th2 immunity .
	manualset3
133920	1	406333	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Optic nerve involvement ( OR 4.30 , 95 % CI 1.50-12 .3 , p = 0.007 ) was associated with a severe initial demyelinating event ( IDE ) , while non-White race ( OR 2.55 , 95 % CI 0.87-7 .49 , p = 0.088 ) , localization to the cerebral hemispheres ( OR 7.94 , 95 % CI 0.86-73 .8 , p = 0.068 ) , or encephalopathy ( OR 8.70 , 95 % CI 0.86-88 .0 , p = 0.067 ) showed a trend towards increased IDE severity .
	manualset3
133921	2	406333	13	NULL	NULL	0	NULL	Optic nerve involvement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Optic nerve involvement ( OR 4.30 , 95 % CI 1.50-12 .3 , p = 0.007 ) was associated with a severe initial demyelinating event ( IDE ) , while non-White race ( OR 2.55 , 95 % CI 0.87-7 .49 , p = 0.088 ) , localization to the cerebral hemispheres ( OR 7.94 , 95 % CI 0.86-73 .8 , p = 0.068 ) , or encephalopathy ( OR 8.70 , 95 % CI 0.86-88 .0 , p = 0.067 ) showed a trend towards increased IDE severity .
	manualset3
133922	3	406333	13	NULL	NULL	0	NULL	OR 4.30	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Optic nerve involvement ( OR 4.30 , 95 % CI 1.50-12 .3 , p = 0.007 ) was associated with a severe initial demyelinating event ( IDE ) , while non-White race ( OR 2.55 , 95 % CI 0.87-7 .49 , p = 0.088 ) , localization to the cerebral hemispheres ( OR 7.94 , 95 % CI 0.86-73 .8 , p = 0.068 ) , or encephalopathy ( OR 8.70 , 95 % CI 0.86-88 .0 , p = 0.067 ) showed a trend towards increased IDE severity .
	manualset3
133923	4	406333	13	NULL	NULL	0	NULL	95 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Optic nerve involvement ( OR 4.30 , 95 % CI 1.50-12 .3 , p = 0.007 ) was associated with a severe initial demyelinating event ( IDE ) , while non-White race ( OR 2.55 , 95 % CI 0.87-7 .49 , p = 0.088 ) , localization to the cerebral hemispheres ( OR 7.94 , 95 % CI 0.86-73 .8 , p = 0.068 ) , or encephalopathy ( OR 8.70 , 95 % CI 0.86-88 .0 , p = 0.067 ) showed a trend towards increased IDE severity .
	manualset3
133924	5	406333	13	NULL	NULL	0	NULL	CI 1.50-12 .3	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Optic nerve involvement ( OR 4.30 , 95 % CI 1.50-12 .3 , p = 0.007 ) was associated with a severe initial demyelinating event ( IDE ) , while non-White race ( OR 2.55 , 95 % CI 0.87-7 .49 , p = 0.088 ) , localization to the cerebral hemispheres ( OR 7.94 , 95 % CI 0.86-73 .8 , p = 0.068 ) , or encephalopathy ( OR 8.70 , 95 % CI 0.86-88 .0 , p = 0.067 ) showed a trend towards increased IDE severity .
	manualset3
133925	6	406333	13	NULL	NULL	0	NULL	p = 0.007 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Optic nerve involvement ( OR 4.30 , 95 % CI 1.50-12 .3 , p = 0.007 ) was associated with a severe initial demyelinating event ( IDE ) , while non-White race ( OR 2.55 , 95 % CI 0.87-7 .49 , p = 0.088 ) , localization to the cerebral hemispheres ( OR 7.94 , 95 % CI 0.86-73 .8 , p = 0.068 ) , or encephalopathy ( OR 8.70 , 95 % CI 0.86-88 .0 , p = 0.067 ) showed a trend towards increased IDE severity .
	manualset3
133926	7	406333	13	NULL	NULL	0	NULL	severe initial demyelinating event ( IDE )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Optic nerve involvement ( OR 4.30 , 95 % CI 1.50-12 .3 , p = 0.007 ) was associated with a severe initial demyelinating event ( IDE ) , while non-White race ( OR 2.55 , 95 % CI 0.87-7 .49 , p = 0.088 ) , localization to the cerebral hemispheres ( OR 7.94 , 95 % CI 0.86-73 .8 , p = 0.068 ) , or encephalopathy ( OR 8.70 , 95 % CI 0.86-88 .0 , p = 0.067 ) showed a trend towards increased IDE severity .
	manualset3
133927	8	406333	13	NULL	NULL	0	NULL	non-White race	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Optic nerve involvement ( OR 4.30 , 95 % CI 1.50-12 .3 , p = 0.007 ) was associated with a severe initial demyelinating event ( IDE ) , while non-White race ( OR 2.55 , 95 % CI 0.87-7 .49 , p = 0.088 ) , localization to the cerebral hemispheres ( OR 7.94 , 95 % CI 0.86-73 .8 , p = 0.068 ) , or encephalopathy ( OR 8.70 , 95 % CI 0.86-88 .0 , p = 0.067 ) showed a trend towards increased IDE severity .
	manualset3
133928	9	406333	13	NULL	NULL	0	NULL	OR 2.55	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Optic nerve involvement ( OR 4.30 , 95 % CI 1.50-12 .3 , p = 0.007 ) was associated with a severe initial demyelinating event ( IDE ) , while non-White race ( OR 2.55 , 95 % CI 0.87-7 .49 , p = 0.088 ) , localization to the cerebral hemispheres ( OR 7.94 , 95 % CI 0.86-73 .8 , p = 0.068 ) , or encephalopathy ( OR 8.70 , 95 % CI 0.86-88 .0 , p = 0.067 ) showed a trend towards increased IDE severity .
	manualset3
133929	10	406333	13	NULL	NULL	0	NULL	95 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Optic nerve involvement ( OR 4.30 , 95 % CI 1.50-12 .3 , p = 0.007 ) was associated with a severe initial demyelinating event ( IDE ) , while non-White race ( OR 2.55 , 95 % CI 0.87-7 .49 , p = 0.088 ) , localization to the cerebral hemispheres ( OR 7.94 , 95 % CI 0.86-73 .8 , p = 0.068 ) , or encephalopathy ( OR 8.70 , 95 % CI 0.86-88 .0 , p = 0.067 ) showed a trend towards increased IDE severity .
	manualset3
133930	11	406333	13	NULL	NULL	0	NULL	CI 0.87-7 .49	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Optic nerve involvement ( OR 4.30 , 95 % CI 1.50-12 .3 , p = 0.007 ) was associated with a severe initial demyelinating event ( IDE ) , while non-White race ( OR 2.55 , 95 % CI 0.87-7 .49 , p = 0.088 ) , localization to the cerebral hemispheres ( OR 7.94 , 95 % CI 0.86-73 .8 , p = 0.068 ) , or encephalopathy ( OR 8.70 , 95 % CI 0.86-88 .0 , p = 0.067 ) showed a trend towards increased IDE severity .
	manualset3
133931	12	406333	13	NULL	NULL	0	NULL	p = 0.088 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Optic nerve involvement ( OR 4.30 , 95 % CI 1.50-12 .3 , p = 0.007 ) was associated with a severe initial demyelinating event ( IDE ) , while non-White race ( OR 2.55 , 95 % CI 0.87-7 .49 , p = 0.088 ) , localization to the cerebral hemispheres ( OR 7.94 , 95 % CI 0.86-73 .8 , p = 0.068 ) , or encephalopathy ( OR 8.70 , 95 % CI 0.86-88 .0 , p = 0.067 ) showed a trend towards increased IDE severity .
	manualset3
133932	13	406333	13	NULL	NULL	0	NULL	localization 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Optic nerve involvement ( OR 4.30 , 95 % CI 1.50-12 .3 , p = 0.007 ) was associated with a severe initial demyelinating event ( IDE ) , while non-White race ( OR 2.55 , 95 % CI 0.87-7 .49 , p = 0.088 ) , localization to the cerebral hemispheres ( OR 7.94 , 95 % CI 0.86-73 .8 , p = 0.068 ) , or encephalopathy ( OR 8.70 , 95 % CI 0.86-88 .0 , p = 0.067 ) showed a trend towards increased IDE severity .
	manualset3
133933	14	406333	13	NULL	NULL	0	NULL	cerebral hemispheres	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Optic nerve involvement ( OR 4.30 , 95 % CI 1.50-12 .3 , p = 0.007 ) was associated with a severe initial demyelinating event ( IDE ) , while non-White race ( OR 2.55 , 95 % CI 0.87-7 .49 , p = 0.088 ) , localization to the cerebral hemispheres ( OR 7.94 , 95 % CI 0.86-73 .8 , p = 0.068 ) , or encephalopathy ( OR 8.70 , 95 % CI 0.86-88 .0 , p = 0.067 ) showed a trend towards increased IDE severity .
	manualset3
133934	15	406333	13	NULL	NULL	0	NULL	OR 7.94	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Optic nerve involvement ( OR 4.30 , 95 % CI 1.50-12 .3 , p = 0.007 ) was associated with a severe initial demyelinating event ( IDE ) , while non-White race ( OR 2.55 , 95 % CI 0.87-7 .49 , p = 0.088 ) , localization to the cerebral hemispheres ( OR 7.94 , 95 % CI 0.86-73 .8 , p = 0.068 ) , or encephalopathy ( OR 8.70 , 95 % CI 0.86-88 .0 , p = 0.067 ) showed a trend towards increased IDE severity .
	manualset3
133935	16	406333	13	NULL	NULL	0	NULL	95 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Optic nerve involvement ( OR 4.30 , 95 % CI 1.50-12 .3 , p = 0.007 ) was associated with a severe initial demyelinating event ( IDE ) , while non-White race ( OR 2.55 , 95 % CI 0.87-7 .49 , p = 0.088 ) , localization to the cerebral hemispheres ( OR 7.94 , 95 % CI 0.86-73 .8 , p = 0.068 ) , or encephalopathy ( OR 8.70 , 95 % CI 0.86-88 .0 , p = 0.067 ) showed a trend towards increased IDE severity .
	manualset3
133936	17	406333	13	NULL	NULL	0	NULL	CI 0.86-73 .8	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Optic nerve involvement ( OR 4.30 , 95 % CI 1.50-12 .3 , p = 0.007 ) was associated with a severe initial demyelinating event ( IDE ) , while non-White race ( OR 2.55 , 95 % CI 0.87-7 .49 , p = 0.088 ) , localization to the cerebral hemispheres ( OR 7.94 , 95 % CI 0.86-73 .8 , p = 0.068 ) , or encephalopathy ( OR 8.70 , 95 % CI 0.86-88 .0 , p = 0.067 ) showed a trend towards increased IDE severity .
	manualset3
133937	18	406333	13	NULL	NULL	0	NULL	p = 0.068 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Optic nerve involvement ( OR 4.30 , 95 % CI 1.50-12 .3 , p = 0.007 ) was associated with a severe initial demyelinating event ( IDE ) , while non-White race ( OR 2.55 , 95 % CI 0.87-7 .49 , p = 0.088 ) , localization to the cerebral hemispheres ( OR 7.94 , 95 % CI 0.86-73 .8 , p = 0.068 ) , or encephalopathy ( OR 8.70 , 95 % CI 0.86-88 .0 , p = 0.067 ) showed a trend towards increased IDE severity .
	manualset3
133938	19	406333	13	NULL	NULL	0	NULL	encephalopathy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Optic nerve involvement ( OR 4.30 , 95 % CI 1.50-12 .3 , p = 0.007 ) was associated with a severe initial demyelinating event ( IDE ) , while non-White race ( OR 2.55 , 95 % CI 0.87-7 .49 , p = 0.088 ) , localization to the cerebral hemispheres ( OR 7.94 , 95 % CI 0.86-73 .8 , p = 0.068 ) , or encephalopathy ( OR 8.70 , 95 % CI 0.86-88 .0 , p = 0.067 ) showed a trend towards increased IDE severity .
	manualset3
133939	20	406333	13	NULL	NULL	0	NULL	OR 8.70	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Optic nerve involvement ( OR 4.30 , 95 % CI 1.50-12 .3 , p = 0.007 ) was associated with a severe initial demyelinating event ( IDE ) , while non-White race ( OR 2.55 , 95 % CI 0.87-7 .49 , p = 0.088 ) , localization to the cerebral hemispheres ( OR 7.94 , 95 % CI 0.86-73 .8 , p = 0.068 ) , or encephalopathy ( OR 8.70 , 95 % CI 0.86-88 .0 , p = 0.067 ) showed a trend towards increased IDE severity .
	manualset3
133940	21	406333	13	NULL	NULL	0	NULL	95 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Optic nerve involvement ( OR 4.30 , 95 % CI 1.50-12 .3 , p = 0.007 ) was associated with a severe initial demyelinating event ( IDE ) , while non-White race ( OR 2.55 , 95 % CI 0.87-7 .49 , p = 0.088 ) , localization to the cerebral hemispheres ( OR 7.94 , 95 % CI 0.86-73 .8 , p = 0.068 ) , or encephalopathy ( OR 8.70 , 95 % CI 0.86-88 .0 , p = 0.067 ) showed a trend towards increased IDE severity .
	manualset3
133941	22	406333	13	NULL	NULL	0	NULL	CI 0.86-88 .0	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Optic nerve involvement ( OR 4.30 , 95 % CI 1.50-12 .3 , p = 0.007 ) was associated with a severe initial demyelinating event ( IDE ) , while non-White race ( OR 2.55 , 95 % CI 0.87-7 .49 , p = 0.088 ) , localization to the cerebral hemispheres ( OR 7.94 , 95 % CI 0.86-73 .8 , p = 0.068 ) , or encephalopathy ( OR 8.70 , 95 % CI 0.86-88 .0 , p = 0.067 ) showed a trend towards increased IDE severity .
	manualset3
133942	23	406333	13	NULL	NULL	0	NULL	p = 0.067	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Optic nerve involvement ( OR 4.30 , 95 % CI 1.50-12 .3 , p = 0.007 ) was associated with a severe initial demyelinating event ( IDE ) , while non-White race ( OR 2.55 , 95 % CI 0.87-7 .49 , p = 0.088 ) , localization to the cerebral hemispheres ( OR 7.94 , 95 % CI 0.86-73 .8 , p = 0.068 ) , or encephalopathy ( OR 8.70 , 95 % CI 0.86-88 .0 , p = 0.067 ) showed a trend towards increased IDE severity .
	manualset3
133943	24	406333	13	NULL	NULL	0	NULL	IDE severity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : Optic nerve involvement ( OR 4.30 , 95 % CI 1.50-12 .3 , p = 0.007 ) was associated with a severe initial demyelinating event ( IDE ) , while non-White race ( OR 2.55 , 95 % CI 0.87-7 .49 , p = 0.088 ) , localization to the cerebral hemispheres ( OR 7.94 , 95 % CI 0.86-73 .8 , p = 0.068 ) , or encephalopathy ( OR 8.70 , 95 % CI 0.86-88 .0 , p = 0.067 ) showed a trend towards increased IDE severity .
	manualset3
133944	1	406334	13	NULL	NULL	0	NULL	mutant IGTP protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A mutant IGTP protein was created that had no detectable complexed GTP , and in both subcellular fractionation and IGTP-green fluorescent protein fusion studies , this mutant also localized to the endoplasmic reticulum .
	manualset3
133945	2	406334	13	NULL	NULL	0	NULL	GTP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A mutant IGTP protein was created that had no detectable complexed GTP , and in both subcellular fractionation and IGTP-green fluorescent protein fusion studies , this mutant also localized to the endoplasmic reticulum .
	manualset3
133946	3	406334	13	NULL	NULL	0	NULL	subcellular fractionation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A mutant IGTP protein was created that had no detectable complexed GTP , and in both subcellular fractionation and IGTP-green fluorescent protein fusion studies , this mutant also localized to the endoplasmic reticulum .
	manualset3
133947	4	406334	13	NULL	NULL	0	NULL	IGTP-green fluorescent protein fusion studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A mutant IGTP protein was created that had no detectable complexed GTP , and in both subcellular fractionation and IGTP-green fluorescent protein fusion studies , this mutant also localized to the endoplasmic reticulum .
	manualset3
133948	5	406334	13	NULL	NULL	0	NULL	mutant	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A mutant IGTP protein was created that had no detectable complexed GTP , and in both subcellular fractionation and IGTP-green fluorescent protein fusion studies , this mutant also localized to the endoplasmic reticulum .
	manualset3
133949	6	406334	13	NULL	NULL	0	NULL	 endoplasmic reticulum	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A mutant IGTP protein was created that had no detectable complexed GTP , and in both subcellular fractionation and IGTP-green fluorescent protein fusion studies , this mutant also localized to the endoplasmic reticulum .
	manualset3
133950	1	406335	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : The TSAb levels significantly decreased only in the remitting group as evidenced by Mc4 assay values at the end of ATD ( 0.96 1.47 , 10.9 26.6 .
	manualset3
133951	2	406335	13	NULL	NULL	0	NULL	TSAb levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : The TSAb levels significantly decreased only in the remitting group as evidenced by Mc4 assay values at the end of ATD ( 0.96 1.47 , 10.9 26.6 .
	manualset3
133952	3	406335	13	NULL	NULL	0	NULL	remitting group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : The TSAb levels significantly decreased only in the remitting group as evidenced by Mc4 assay values at the end of ATD ( 0.96 1.47 , 10.9 26.6 .
	manualset3
133953	4	406335	13	NULL	NULL	0	NULL	Mc4 assay values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : The TSAb levels significantly decreased only in the remitting group as evidenced by Mc4 assay values at the end of ATD ( 0.96 1.47 , 10.9 26.6 .
	manualset3
133954	5	406335	13	NULL	NULL	0	NULL	end	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : The TSAb levels significantly decreased only in the remitting group as evidenced by Mc4 assay values at the end of ATD ( 0.96 1.47 , 10.9 26.6 .
	manualset3
133955	6	406335	13	NULL	NULL	0	NULL	ATD 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : The TSAb levels significantly decreased only in the remitting group as evidenced by Mc4 assay values at the end of ATD ( 0.96 1.47 , 10.9 26.6 .
	manualset3
133956	7	406335	13	NULL	NULL	0	NULL	0.96 1.47 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : The TSAb levels significantly decreased only in the remitting group as evidenced by Mc4 assay values at the end of ATD ( 0.96 1.47 , 10.9 26.6 .
	manualset3
133957	8	406335	13	NULL	NULL	0	NULL	10.9 26.6 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : The TSAb levels significantly decreased only in the remitting group as evidenced by Mc4 assay values at the end of ATD ( 0.96 1.47 , 10.9 26.6 .
	manualset3
133958	1	406336	13	NULL	NULL	0	NULL	Results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : The average age was 22 + / -4.9 years in the different sports ( canoeing , pentathlon , handball , basketball , volleyball , weight-lifting ) .
	manualset3
133959	2	406336	13	NULL	NULL	0	NULL	average age 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : The average age was 22 + / -4.9 years in the different sports ( canoeing , pentathlon , handball , basketball , volleyball , weight-lifting ) .
	manualset3
133960	3	406336	13	NULL	NULL	0	NULL	22 + / -4.9 years 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : The average age was 22 + / -4.9 years in the different sports ( canoeing , pentathlon , handball , basketball , volleyball , weight-lifting ) .
	manualset3
133961	4	406336	13	NULL	NULL	0	NULL	sports	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : The average age was 22 + / -4.9 years in the different sports ( canoeing , pentathlon , handball , basketball , volleyball , weight-lifting ) .
	manualset3
133962	5	406336	13	NULL	NULL	0	NULL	canoeing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : The average age was 22 + / -4.9 years in the different sports ( canoeing , pentathlon , handball , basketball , volleyball , weight-lifting ) .
	manualset3
133963	6	406336	13	NULL	NULL	0	NULL	pentathlon	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : The average age was 22 + / -4.9 years in the different sports ( canoeing , pentathlon , handball , basketball , volleyball , weight-lifting ) .
	manualset3
133964	7	406336	13	NULL	NULL	0	NULL	handball	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : The average age was 22 + / -4.9 years in the different sports ( canoeing , pentathlon , handball , basketball , volleyball , weight-lifting ) .
	manualset3
133965	8	406336	13	NULL	NULL	0	NULL	basketball	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : The average age was 22 + / -4.9 years in the different sports ( canoeing , pentathlon , handball , basketball , volleyball , weight-lifting ) .
	manualset3
133966	9	406336	13	NULL	NULL	0	NULL	volleyball	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : The average age was 22 + / -4.9 years in the different sports ( canoeing , pentathlon , handball , basketball , volleyball , weight-lifting ) .
	manualset3
133967	10	406336	13	NULL	NULL	0	NULL	weight-lifting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : The average age was 22 + / -4.9 years in the different sports ( canoeing , pentathlon , handball , basketball , volleyball , weight-lifting ) .
	manualset3
134041	1	406337	13	NULL	NULL	0	NULL	Results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : The high coefficient of correlation of ferritin values between the new monoclonal assay and conventional assay indicated that this monoclonal assay system was useful in measuring serum ferritin .
	manualset3
134042	2	406337	13	NULL	NULL	NULL	NULL	coefficient of correlation	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Results : The high coefficient of correlation of ferritin values between the new monoclonal assay and conventional assay indicated that this monoclonal assay system was useful in measuring serum ferritin .
	manualset3
134044	4	406337	13	NULL	NULL	0	NULL	ferritin values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : The high coefficient of correlation of ferritin values between the new monoclonal assay and conventional assay indicated that this monoclonal assay system was useful in measuring serum ferritin .
	manualset3
134045	5	406337	13	NULL	NULL	0	NULL	monoclonal assay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : The high coefficient of correlation of ferritin values between the new monoclonal assay and conventional assay indicated that this monoclonal assay system was useful in measuring serum ferritin .
	manualset3
134046	6	406337	13	NULL	NULL	0	NULL	conventional assay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : The high coefficient of correlation of ferritin values between the new monoclonal assay and conventional assay indicated that this monoclonal assay system was useful in measuring serum ferritin .
	manualset3
134047	7	406337	13	NULL	NULL	0	NULL	monoclonal assay system	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : The high coefficient of correlation of ferritin values between the new monoclonal assay and conventional assay indicated that this monoclonal assay system was useful in measuring serum ferritin .
	manualset3
134048	8	406337	13	NULL	NULL	0	NULL	serum ferritin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Results : The high coefficient of correlation of ferritin values between the new monoclonal assay and conventional assay indicated that this monoclonal assay system was useful in measuring serum ferritin .
	manualset3
134049	1	406338	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Improved survival was associated with being in the high-scoring group ( high vs low scores : 5-year OS , 40 % vs 17 % , P & lt ; .001 ) , and results were reproduced in the validation datasets ( P & lt ; .05 ) .
	manualset3
134050	2	406338	13	NULL	NULL	0	NULL	survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Improved survival was associated with being in the high-scoring group ( high vs low scores : 5-year OS , 40 % vs 17 % , P & lt ; .001 ) , and results were reproduced in the validation datasets ( P & lt ; .05 ) .
	manualset3
134051	3	406338	13	NULL	NULL	0	NULL	high-scoring group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Improved survival was associated with being in the high-scoring group ( high vs low scores : 5-year OS , 40 % vs 17 % , P & lt ; .001 ) , and results were reproduced in the validation datasets ( P & lt ; .05 ) .
	manualset3
134052	4	406338	13	NULL	NULL	0	NULL	high vs low scores	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Improved survival was associated with being in the high-scoring group ( high vs low scores : 5-year OS , 40 % vs 17 % , P & lt ; .001 ) , and results were reproduced in the validation datasets ( P & lt ; .05 ) .
	manualset3
134053	5	406338	13	NULL	NULL	0	NULL	5-year OS	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Improved survival was associated with being in the high-scoring group ( high vs low scores : 5-year OS , 40 % vs 17 % , P & lt ; .001 ) , and results were reproduced in the validation datasets ( P & lt ; .05 ) .
	manualset3
134054	6	406338	13	NULL	NULL	0	NULL	40 % vs 17 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Improved survival was associated with being in the high-scoring group ( high vs low scores : 5-year OS , 40 % vs 17 % , P & lt ; .001 ) , and results were reproduced in the validation datasets ( P & lt ; .05 ) .
	manualset3
134055	7	406338	13	NULL	NULL	0	NULL	P & lt ; .001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Improved survival was associated with being in the high-scoring group ( high vs low scores : 5-year OS , 40 % vs 17 % , P & lt ; .001 ) , and results were reproduced in the validation datasets ( P & lt ; .05 ) .
	manualset3
134056	8	406338	13	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Improved survival was associated with being in the high-scoring group ( high vs low scores : 5-year OS , 40 % vs 17 % , P & lt ; .001 ) , and results were reproduced in the validation datasets ( P & lt ; .05 ) .
	manualset3
134057	9	406338	13	NULL	NULL	0	NULL	validation datasets	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Improved survival was associated with being in the high-scoring group ( high vs low scores : 5-year OS , 40 % vs 17 % , P & lt ; .001 ) , and results were reproduced in the validation datasets ( P & lt ; .05 ) .
	manualset3
134058	10	406338	13	NULL	NULL	0	NULL	P & lt ; .05 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Improved survival was associated with being in the high-scoring group ( high vs low scores : 5-year OS , 40 % vs 17 % , P & lt ; .001 ) , and results were reproduced in the validation datasets ( P & lt ; .05 ) .
	manualset3
134059	1	406339	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Of the 405 patients studied , 44 % ( 59/134 ) of girls had undergone surgery at 1 year compared with 70 % ( 189/271 ) of boys ( ( 2 ) = 24.97 ; p & lt ; 0.001 ) .
	manualset3
134060	2	406339	13	NULL	NULL	0	NULL	 405 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Of the 405 patients studied , 44 % ( 59/134 ) of girls had undergone surgery at 1 year compared with 70 % ( 189/271 ) of boys ( ( 2 ) = 24.97 ; p & lt ; 0.001 ) .
	manualset3
134061	3	406339	13	NULL	NULL	0	NULL	44 % ( 59/134 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Of the 405 patients studied , 44 % ( 59/134 ) of girls had undergone surgery at 1 year compared with 70 % ( 189/271 ) of boys ( ( 2 ) = 24.97 ; p & lt ; 0.001 ) .
	manualset3
134062	4	406339	13	NULL	NULL	0	NULL	girls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Of the 405 patients studied , 44 % ( 59/134 ) of girls had undergone surgery at 1 year compared with 70 % ( 189/271 ) of boys ( ( 2 ) = 24.97 ; p & lt ; 0.001 ) .
	manualset3
134063	5	406339	13	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Of the 405 patients studied , 44 % ( 59/134 ) of girls had undergone surgery at 1 year compared with 70 % ( 189/271 ) of boys ( ( 2 ) = 24.97 ; p & lt ; 0.001 ) .
	manualset3
134064	6	406339	13	NULL	NULL	0	NULL	1 year	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Of the 405 patients studied , 44 % ( 59/134 ) of girls had undergone surgery at 1 year compared with 70 % ( 189/271 ) of boys ( ( 2 ) = 24.97 ; p & lt ; 0.001 ) .
	manualset3
134065	7	406339	13	NULL	NULL	0	NULL	70 % ( 189/271 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Of the 405 patients studied , 44 % ( 59/134 ) of girls had undergone surgery at 1 year compared with 70 % ( 189/271 ) of boys ( ( 2 ) = 24.97 ; p & lt ; 0.001 ) .
	manualset3
134066	8	406339	13	NULL	NULL	0	NULL	boys 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Of the 405 patients studied , 44 % ( 59/134 ) of girls had undergone surgery at 1 year compared with 70 % ( 189/271 ) of boys ( ( 2 ) = 24.97 ; p & lt ; 0.001 ) .
	manualset3
134067	9	406339	13	NULL	NULL	0	NULL	( 2 ) = 24.97 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Of the 405 patients studied , 44 % ( 59/134 ) of girls had undergone surgery at 1 year compared with 70 % ( 189/271 ) of boys ( ( 2 ) = 24.97 ; p & lt ; 0.001 ) .
	manualset3
134068	10	406339	13	NULL	NULL	0	NULL	p & lt ; 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Of the 405 patients studied , 44 % ( 59/134 ) of girls had undergone surgery at 1 year compared with 70 % ( 189/271 ) of boys ( ( 2 ) = 24.97 ; p & lt ; 0.001 ) .
	manualset3
134069	1	406340	13	NULL	NULL	0	NULL	Results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Patients with low systemic BMD showed higher subsidence of the femoral stem during the first 3 months after surgery than did those with normal BMD ( difference = 0.6 , 95 % CI : 0.1-1 .1 ; p = 0.03 ) .
	manualset3
134070	2	406340	13	NULL	NULL	0	NULL	Patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Patients with low systemic BMD showed higher subsidence of the femoral stem during the first 3 months after surgery than did those with normal BMD ( difference = 0.6 , 95 % CI : 0.1-1 .1 ; p = 0.03 ) .
	manualset3
134071	3	406340	13	NULL	NULL	0	NULL	low systemic BMD	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Patients with low systemic BMD showed higher subsidence of the femoral stem during the first 3 months after surgery than did those with normal BMD ( difference = 0.6 , 95 % CI : 0.1-1 .1 ; p = 0.03 ) .
	manualset3
134072	4	406340	13	NULL	NULL	0	NULL	subsidence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Patients with low systemic BMD showed higher subsidence of the femoral stem during the first 3 months after surgery than did those with normal BMD ( difference = 0.6 , 95 % CI : 0.1-1 .1 ; p = 0.03 ) .
	manualset3
134073	5	406340	13	NULL	NULL	0	NULL	femoral stem	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Patients with low systemic BMD showed higher subsidence of the femoral stem during the first 3 months after surgery than did those with normal BMD ( difference = 0.6 , 95 % CI : 0.1-1 .1 ; p = 0.03 ) .
	manualset3
134074	6	406340	13	NULL	NULL	0	NULL	3 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Patients with low systemic BMD showed higher subsidence of the femoral stem during the first 3 months after surgery than did those with normal BMD ( difference = 0.6 , 95 % CI : 0.1-1 .1 ; p = 0.03 ) .
	manualset3
134075	7	406340	13	NULL	NULL	0	NULL	surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Patients with low systemic BMD showed higher subsidence of the femoral stem during the first 3 months after surgery than did those with normal BMD ( difference = 0.6 , 95 % CI : 0.1-1 .1 ; p = 0.03 ) .
	manualset3
134076	8	406340	13	NULL	NULL	0	NULL	normal BMD	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Patients with low systemic BMD showed higher subsidence of the femoral stem during the first 3 months after surgery than did those with normal BMD ( difference = 0.6 , 95 % CI : 0.1-1 .1 ; p = 0.03 ) .
	manualset3
134077	9	406340	13	NULL	NULL	0	NULL	difference = 0.6	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Patients with low systemic BMD showed higher subsidence of the femoral stem during the first 3 months after surgery than did those with normal BMD ( difference = 0.6 , 95 % CI : 0.1-1 .1 ; p = 0.03 ) .
	manualset3
134078	10	406340	13	NULL	NULL	0	NULL	95 % CI : 0.1-1 .1 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Patients with low systemic BMD showed higher subsidence of the femoral stem during the first 3 months after surgery than did those with normal BMD ( difference = 0.6 , 95 % CI : 0.1-1 .1 ; p = 0.03 ) .
	manualset3
134079	11	406340	13	NULL	NULL	0	NULL	p = 0.03 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results Patients with low systemic BMD showed higher subsidence of the femoral stem during the first 3 months after surgery than did those with normal BMD ( difference = 0.6 , 95 % CI : 0.1-1 .1 ; p = 0.03 ) .
	manualset3
134080	1	406341	13	NULL	NULL	0	NULL	Results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results are discussed regarding the implications for transfer , generalization , and procedural application .
	manualset3
134081	2	406341	13	NULL	NULL	0	NULL	implications 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results are discussed regarding the implications for transfer , generalization , and procedural application .
	manualset3
134082	3	406341	13	NULL	NULL	0	NULL	transfer	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results are discussed regarding the implications for transfer , generalization , and procedural application .
	manualset3
134083	4	406341	13	NULL	NULL	0	NULL	generalization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results are discussed regarding the implications for transfer , generalization , and procedural application .
	manualset3
134084	5	406341	13	NULL	NULL	0	NULL	procedural application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results are discussed regarding the implications for transfer , generalization , and procedural application .
	manualset3
134085	1	406342	13	NULL	NULL	0	NULL	mutation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A mutation of an insertion of 4 bp in the gene for the alpha subunit of pyruvate dehydrogenase ( E1 alpha ) was found in a female with pyruvate dehydrogenase deficiency due to the rapid degradation of alpha and beta subunit proteins of pyruvate dehydrogenase .
	manualset3
134086	2	406342	13	NULL	NULL	0	NULL	insertion 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A mutation of an insertion of 4 bp in the gene for the alpha subunit of pyruvate dehydrogenase ( E1 alpha ) was found in a female with pyruvate dehydrogenase deficiency due to the rapid degradation of alpha and beta subunit proteins of pyruvate dehydrogenase .
	manualset3
134087	3	406342	13	NULL	NULL	0	NULL	4 bp	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A mutation of an insertion of 4 bp in the gene for the alpha subunit of pyruvate dehydrogenase ( E1 alpha ) was found in a female with pyruvate dehydrogenase deficiency due to the rapid degradation of alpha and beta subunit proteins of pyruvate dehydrogenase .
	manualset3
134088	4	406342	13	NULL	NULL	0	NULL	gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A mutation of an insertion of 4 bp in the gene for the alpha subunit of pyruvate dehydrogenase ( E1 alpha ) was found in a female with pyruvate dehydrogenase deficiency due to the rapid degradation of alpha and beta subunit proteins of pyruvate dehydrogenase .
	manualset3
134089	5	406342	13	NULL	NULL	NULL	NULL	alpha subunit of pyruvate dehydrogenase ( E1 alpha )	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A mutation of an insertion of 4 bp in the gene for the alpha subunit of pyruvate dehydrogenase ( E1 alpha ) was found in a female with pyruvate dehydrogenase deficiency due to the rapid degradation of alpha and beta subunit proteins of pyruvate dehydrogenase .
	manualset3
134090	6	406342	13	NULL	NULL	0	NULL	female	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A mutation of an insertion of 4 bp in the gene for the alpha subunit of pyruvate dehydrogenase ( E1 alpha ) was found in a female with pyruvate dehydrogenase deficiency due to the rapid degradation of alpha and beta subunit proteins of pyruvate dehydrogenase .
	manualset3
134091	7	406342	13	NULL	NULL	0	NULL	pyruvate dehydrogenase deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A mutation of an insertion of 4 bp in the gene for the alpha subunit of pyruvate dehydrogenase ( E1 alpha ) was found in a female with pyruvate dehydrogenase deficiency due to the rapid degradation of alpha and beta subunit proteins of pyruvate dehydrogenase .
	manualset3
134092	8	406342	13	NULL	NULL	0	NULL	degradation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A mutation of an insertion of 4 bp in the gene for the alpha subunit of pyruvate dehydrogenase ( E1 alpha ) was found in a female with pyruvate dehydrogenase deficiency due to the rapid degradation of alpha and beta subunit proteins of pyruvate dehydrogenase .
	manualset3
134093	9	406342	13	NULL	NULL	0	NULL	alpha subunit protein of pyruvate dehydrogenase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A mutation of an insertion of 4 bp in the gene for the alpha subunit of pyruvate dehydrogenase ( E1 alpha ) was found in a female with pyruvate dehydrogenase deficiency due to the rapid degradation of alpha and beta subunit proteins of pyruvate dehydrogenase .
	manualset3
134094	10	406342	13	NULL	NULL	0	NULL	beta subunit protein of pyruvate dehydrogenase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A mutation of an insertion of 4 bp in the gene for the alpha subunit of pyruvate dehydrogenase ( E1 alpha ) was found in a female with pyruvate dehydrogenase deficiency due to the rapid degradation of alpha and beta subunit proteins of pyruvate dehydrogenase .
	manualset3
134095	1	406343	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrate that smoking ban in public places is widely respected and that the application of the law had a very positive impact on the quality of life and health of workers and general population .
	manualset3
134096	2	406343	13	NULL	NULL	0	NULL	ban 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrate that smoking ban in public places is widely respected and that the application of the law had a very positive impact on the quality of life and health of workers and general population .
	manualset3
134097	3	406343	13	NULL	NULL	0	NULL	public places	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrate that smoking ban in public places is widely respected and that the application of the law had a very positive impact on the quality of life and health of workers and general population .
	manualset3
134098	4	406343	13	NULL	NULL	0	NULL	application 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrate that smoking ban in public places is widely respected and that the application of the law had a very positive impact on the quality of life and health of workers and general population .
	manualset3
134099	5	406343	13	NULL	NULL	0	NULL	law	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrate that smoking ban in public places is widely respected and that the application of the law had a very positive impact on the quality of life and health of workers and general population .
	manualset3
134100	6	406343	13	NULL	NULL	0	NULL	impact 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrate that smoking ban in public places is widely respected and that the application of the law had a very positive impact on the quality of life and health of workers and general population .
	manualset3
134101	7	406343	13	NULL	NULL	0	NULL	quality of life	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrate that smoking ban in public places is widely respected and that the application of the law had a very positive impact on the quality of life and health of workers and general population .
	manualset3
134102	8	406343	13	NULL	NULL	0	NULL	health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrate that smoking ban in public places is widely respected and that the application of the law had a very positive impact on the quality of life and health of workers and general population .
	manualset3
134103	9	406343	13	NULL	NULL	0	NULL	workers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrate that smoking ban in public places is widely respected and that the application of the law had a very positive impact on the quality of life and health of workers and general population .
	manualset3
134104	10	406343	13	NULL	NULL	0	NULL	general population 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrate that smoking ban in public places is widely respected and that the application of the law had a very positive impact on the quality of life and health of workers and general population .
	manualset3
134105	1	406344	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrate that the affinities of each collagen for syndecan-1 and low-M ( r ) heparin were similar , and followed the order : type V ) ) type IV approximately type III approximately type I ) type VI ) ) type II , and ranged in Kd from approximately 10 ( -8 ) to approximately 3 x 10 ( -6 ) M. These data suggest that syndecan-1 and heparin may contain similar collagen-binding determinants .
	manualset3
134106	2	406344	13	NULL	NULL	0	NULL	affinities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrate that the affinities of each collagen for syndecan-1 and low-M ( r ) heparin were similar , and followed the order : type V ) ) type IV approximately type III approximately type I ) type VI ) ) type II , and ranged in Kd from approximately 10 ( -8 ) to approximately 3 x 10 ( -6 ) M. These data suggest that syndecan-1 and heparin may contain similar collagen-binding determinants .
	manualset3
134107	3	406344	13	NULL	NULL	0	NULL	collagen 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrate that the affinities of each collagen for syndecan-1 and low-M ( r ) heparin were similar , and followed the order : type V ) ) type IV approximately type III approximately type I ) type VI ) ) type II , and ranged in Kd from approximately 10 ( -8 ) to approximately 3 x 10 ( -6 ) M. These data suggest that syndecan-1 and heparin may contain similar collagen-binding determinants .
	manualset3
134108	4	406344	13	NULL	NULL	0	NULL	syndecan-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrate that the affinities of each collagen for syndecan-1 and low-M ( r ) heparin were similar , and followed the order : type V ) ) type IV approximately type III approximately type I ) type VI ) ) type II , and ranged in Kd from approximately 10 ( -8 ) to approximately 3 x 10 ( -6 ) M. These data suggest that syndecan-1 and heparin may contain similar collagen-binding determinants .
	manualset3
134109	5	406344	13	NULL	NULL	0	NULL	low-M ( r ) heparin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrate that the affinities of each collagen for syndecan-1 and low-M ( r ) heparin were similar , and followed the order : type V ) ) type IV approximately type III approximately type I ) type VI ) ) type II , and ranged in Kd from approximately 10 ( -8 ) to approximately 3 x 10 ( -6 ) M. These data suggest that syndecan-1 and heparin may contain similar collagen-binding determinants .
	manualset3
134110	6	406344	13	NULL	NULL	0	NULL	order	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrate that the affinities of each collagen for syndecan-1 and low-M ( r ) heparin were similar , and followed the order : type V ) ) type IV approximately type III approximately type I ) type VI ) ) type II , and ranged in Kd from approximately 10 ( -8 ) to approximately 3 x 10 ( -6 ) M. These data suggest that syndecan-1 and heparin may contain similar collagen-binding determinants .
	manualset3
134111	7	406344	13	NULL	NULL	0	NULL	type V	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrate that the affinities of each collagen for syndecan-1 and low-M ( r ) heparin were similar , and followed the order : type V ) ) type IV approximately type III approximately type I ) type VI ) ) type II , and ranged in Kd from approximately 10 ( -8 ) to approximately 3 x 10 ( -6 ) M. These data suggest that syndecan-1 and heparin may contain similar collagen-binding determinants .
	manualset3
134112	8	406344	13	NULL	NULL	0	NULL	type IV 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrate that the affinities of each collagen for syndecan-1 and low-M ( r ) heparin were similar , and followed the order : type V ) ) type IV approximately type III approximately type I ) type VI ) ) type II , and ranged in Kd from approximately 10 ( -8 ) to approximately 3 x 10 ( -6 ) M. These data suggest that syndecan-1 and heparin may contain similar collagen-binding determinants .
	manualset3
134113	9	406344	13	NULL	NULL	0	NULL	type III	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrate that the affinities of each collagen for syndecan-1 and low-M ( r ) heparin were similar , and followed the order : type V ) ) type IV approximately type III approximately type I ) type VI ) ) type II , and ranged in Kd from approximately 10 ( -8 ) to approximately 3 x 10 ( -6 ) M. These data suggest that syndecan-1 and heparin may contain similar collagen-binding determinants .
	manualset3
134114	10	406344	13	NULL	NULL	0	NULL	type I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrate that the affinities of each collagen for syndecan-1 and low-M ( r ) heparin were similar , and followed the order : type V ) ) type IV approximately type III approximately type I ) type VI ) ) type II , and ranged in Kd from approximately 10 ( -8 ) to approximately 3 x 10 ( -6 ) M. These data suggest that syndecan-1 and heparin may contain similar collagen-binding determinants .
	manualset3
134115	11	406344	13	NULL	NULL	0	NULL	type VI	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrate that the affinities of each collagen for syndecan-1 and low-M ( r ) heparin were similar , and followed the order : type V ) ) type IV approximately type III approximately type I ) type VI ) ) type II , and ranged in Kd from approximately 10 ( -8 ) to approximately 3 x 10 ( -6 ) M. These data suggest that syndecan-1 and heparin may contain similar collagen-binding determinants .
	manualset3
134116	12	406344	13	NULL	NULL	0	NULL	type II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrate that the affinities of each collagen for syndecan-1 and low-M ( r ) heparin were similar , and followed the order : type V ) ) type IV approximately type III approximately type I ) type VI ) ) type II , and ranged in Kd from approximately 10 ( -8 ) to approximately 3 x 10 ( -6 ) M. These data suggest that syndecan-1 and heparin may contain similar collagen-binding determinants .
	manualset3
134117	13	406344	13	NULL	NULL	0	NULL	Kd	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrate that the affinities of each collagen for syndecan-1 and low-M ( r ) heparin were similar , and followed the order : type V ) ) type IV approximately type III approximately type I ) type VI ) ) type II , and ranged in Kd from approximately 10 ( -8 ) to approximately 3 x 10 ( -6 ) M. These data suggest that syndecan-1 and heparin may contain similar collagen-binding determinants .
	manualset3
134118	14	406344	13	NULL	NULL	0	NULL	approximately 10 ( -8 ) to approximately 3 x 10 ( -6 ) M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrate that the affinities of each collagen for syndecan-1 and low-M ( r ) heparin were similar , and followed the order : type V ) ) type IV approximately type III approximately type I ) type VI ) ) type II , and ranged in Kd from approximately 10 ( -8 ) to approximately 3 x 10 ( -6 ) M. These data suggest that syndecan-1 and heparin may contain similar collagen-binding determinants .
	manualset3
134119	15	406344	13	NULL	NULL	0	NULL	data 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrate that the affinities of each collagen for syndecan-1 and low-M ( r ) heparin were similar , and followed the order : type V ) ) type IV approximately type III approximately type I ) type VI ) ) type II , and ranged in Kd from approximately 10 ( -8 ) to approximately 3 x 10 ( -6 ) M. These data suggest that syndecan-1 and heparin may contain similar collagen-binding determinants .
	manualset3
134120	16	406344	13	NULL	NULL	0	NULL	syndecan-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrate that the affinities of each collagen for syndecan-1 and low-M ( r ) heparin were similar , and followed the order : type V ) ) type IV approximately type III approximately type I ) type VI ) ) type II , and ranged in Kd from approximately 10 ( -8 ) to approximately 3 x 10 ( -6 ) M. These data suggest that syndecan-1 and heparin may contain similar collagen-binding determinants .
	manualset3
134121	17	406344	13	NULL	NULL	0	NULL	heparin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrate that the affinities of each collagen for syndecan-1 and low-M ( r ) heparin were similar , and followed the order : type V ) ) type IV approximately type III approximately type I ) type VI ) ) type II , and ranged in Kd from approximately 10 ( -8 ) to approximately 3 x 10 ( -6 ) M. These data suggest that syndecan-1 and heparin may contain similar collagen-binding determinants .
	manualset3
134122	18	406344	13	NULL	NULL	0	NULL	determinants 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrate that the affinities of each collagen for syndecan-1 and low-M ( r ) heparin were similar , and followed the order : type V ) ) type IV approximately type III approximately type I ) type VI ) ) type II , and ranged in Kd from approximately 10 ( -8 ) to approximately 3 x 10 ( -6 ) M. These data suggest that syndecan-1 and heparin may contain similar collagen-binding determinants .
	manualset3
134123	1	406345	13	NULL	NULL	0	NULL	Results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrating the effectiveness of this method , obtained with Monte Carlo techniques , show that the visibility depth can be increased by as much as a mean free path .
	manualset3
134124	2	406345	13	NULL	NULL	0	NULL	effectiveness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrating the effectiveness of this method , obtained with Monte Carlo techniques , show that the visibility depth can be increased by as much as a mean free path .
	manualset3
134125	3	406345	13	NULL	NULL	NULL	NULL	method	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Results demonstrating the effectiveness of this method , obtained with Monte Carlo techniques , show that the visibility depth can be increased by as much as a mean free path .
	manualset3
134126	4	406345	13	NULL	NULL	0	NULL	Monte Carlo techniques	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrating the effectiveness of this method , obtained with Monte Carlo techniques , show that the visibility depth can be increased by as much as a mean free path .
	manualset3
134127	5	406345	13	NULL	NULL	0	NULL	visibility depth	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrating the effectiveness of this method , obtained with Monte Carlo techniques , show that the visibility depth can be increased by as much as a mean free path .
	manualset3
134128	6	406345	13	NULL	NULL	0	NULL	mean free path 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results demonstrating the effectiveness of this method , obtained with Monte Carlo techniques , show that the visibility depth can be increased by as much as a mean free path .
	manualset3
134129	1	406346	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results extend the literature on the associations between adaptive style and self-report instruments and indicate that ( similar to self-reported measures of distress ) self-reported hope may be subject to social desirability bias .
	manualset3
134130	2	406346	13	NULL	NULL	0	NULL	literature 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results extend the literature on the associations between adaptive style and self-report instruments and indicate that ( similar to self-reported measures of distress ) self-reported hope may be subject to social desirability bias .
	manualset3
134131	3	406346	13	NULL	NULL	0	NULL	associations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Results extend the literature on the associations between adaptive style and self-report instruments and indicate that ( similar to self-reported measures of distress ) self-reported hope may be subject to social desirability bias .
	manualset3
134132	4	406346	13	NULL	NULL	0	NULL	adaptive style	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results extend the literature on the associations between adaptive style and self-report instruments and indicate that ( similar to self-reported measures of distress ) self-reported hope may be subject to social desirability bias .
	manualset3
134133	5	406346	13	NULL	NULL	0	NULL	self-report instruments	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Results extend the literature on the associations between adaptive style and self-report instruments and indicate that ( similar to self-reported measures of distress ) self-reported hope may be subject to social desirability bias .
	manualset3
134134	6	406346	13	NULL	NULL	0	NULL	measures 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results extend the literature on the associations between adaptive style and self-report instruments and indicate that ( similar to self-reported measures of distress ) self-reported hope may be subject to social desirability bias .
	manualset3
134135	7	406346	13	NULL	NULL	0	NULL	distress 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results extend the literature on the associations between adaptive style and self-report instruments and indicate that ( similar to self-reported measures of distress ) self-reported hope may be subject to social desirability bias .
	manualset3
134136	8	406346	13	NULL	NULL	0	NULL	hope	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results extend the literature on the associations between adaptive style and self-report instruments and indicate that ( similar to self-reported measures of distress ) self-reported hope may be subject to social desirability bias .
	manualset3
134138	10	406346	13	NULL	NULL	0	NULL	social desirability bias	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results extend the literature on the associations between adaptive style and self-report instruments and indicate that ( similar to self-reported measures of distress ) self-reported hope may be subject to social desirability bias .
	manualset3
134139	1	406347	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from Section 2.2.1 revealed that although rats detected a change in context , the learning was not context specific .
	manualset3
134140	2	406347	13	NULL	NULL	0	NULL	Section 2.2.1	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from Section 2.2.1 revealed that although rats detected a change in context , the learning was not context specific .
	manualset3
134141	3	406347	13	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from Section 2.2.1 revealed that although rats detected a change in context , the learning was not context specific .
	manualset3
134142	4	406347	13	NULL	NULL	0	NULL	change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from Section 2.2.1 revealed that although rats detected a change in context , the learning was not context specific .
	manualset3
134143	5	406347	13	NULL	NULL	0	NULL	context	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from Section 2.2.1 revealed that although rats detected a change in context , the learning was not context specific .
	manualset3
134144	6	406347	13	NULL	NULL	0	NULL	learning 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from Section 2.2.1 revealed that although rats detected a change in context , the learning was not context specific .
	manualset3
134145	7	406347	13	NULL	NULL	0	NULL	context	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from Section 2.2.1 revealed that although rats detected a change in context , the learning was not context specific .
	manualset3
134146	1	406348	13	NULL	NULL	0	NULL	binding site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A narrow binding site of the p68 was revealed using synthetic oligonucleotides .
	manualset3
134147	2	406348	13	NULL	NULL	0	NULL	p68	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A narrow binding site of the p68 was revealed using synthetic oligonucleotides .
	manualset3
134148	3	406348	13	NULL	NULL	0	NULL	synthetic oligonucleotides	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A narrow binding site of the p68 was revealed using synthetic oligonucleotides .
	manualset3
134149	1	406349	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from immunoblot assay and EMSA revealed the modulation of curcumin on the expression of androgen receptor and androgen receptor binding activity on androgen response element of PSA gene .
	manualset3
134150	2	406349	13	NULL	NULL	0	NULL	immunoblot assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from immunoblot assay and EMSA revealed the modulation of curcumin on the expression of androgen receptor and androgen receptor binding activity on androgen response element of PSA gene .
	manualset3
134151	3	406349	13	NULL	NULL	0	NULL	EMSA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from immunoblot assay and EMSA revealed the modulation of curcumin on the expression of androgen receptor and androgen receptor binding activity on androgen response element of PSA gene .
	manualset3
134152	4	406349	13	NULL	NULL	0	NULL	modulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from immunoblot assay and EMSA revealed the modulation of curcumin on the expression of androgen receptor and androgen receptor binding activity on androgen response element of PSA gene .
	manualset3
134153	5	406349	13	NULL	NULL	0	NULL	curcumin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from immunoblot assay and EMSA revealed the modulation of curcumin on the expression of androgen receptor and androgen receptor binding activity on androgen response element of PSA gene .
	manualset3
134154	6	406349	13	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from immunoblot assay and EMSA revealed the modulation of curcumin on the expression of androgen receptor and androgen receptor binding activity on androgen response element of PSA gene .
	manualset3
134155	7	406349	13	NULL	NULL	0	NULL	androgen receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from immunoblot assay and EMSA revealed the modulation of curcumin on the expression of androgen receptor and androgen receptor binding activity on androgen response element of PSA gene .
	manualset3
134156	8	406349	13	NULL	NULL	0	NULL	androgen receptor binding activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from immunoblot assay and EMSA revealed the modulation of curcumin on the expression of androgen receptor and androgen receptor binding activity on androgen response element of PSA gene .
	manualset3
134157	9	406349	13	NULL	NULL	0	NULL	androgen response element	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from immunoblot assay and EMSA revealed the modulation of curcumin on the expression of androgen receptor and androgen receptor binding activity on androgen response element of PSA gene .
	manualset3
134158	10	406349	13	NULL	NULL	0	NULL	PSA gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from immunoblot assay and EMSA revealed the modulation of curcumin on the expression of androgen receptor and androgen receptor binding activity on androgen response element of PSA gene .
	manualset3
134159	1	406350	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from national telephone surveys suggest higher prevalence of overweight among Veterans compared with demographically similar non-Veterans , based on self-reported height and weight .
	manualset3
134160	2	406350	13	NULL	NULL	0	NULL	national telephone surveys	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from national telephone surveys suggest higher prevalence of overweight among Veterans compared with demographically similar non-Veterans , based on self-reported height and weight .
	manualset3
134161	3	406350	13	NULL	NULL	0	NULL	prevalence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from national telephone surveys suggest higher prevalence of overweight among Veterans compared with demographically similar non-Veterans , based on self-reported height and weight .
	manualset3
134162	4	406350	13	NULL	NULL	0	NULL	overweight 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from national telephone surveys suggest higher prevalence of overweight among Veterans compared with demographically similar non-Veterans , based on self-reported height and weight .
	manualset3
134163	5	406350	13	NULL	NULL	0	NULL	Veterans	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from national telephone surveys suggest higher prevalence of overweight among Veterans compared with demographically similar non-Veterans , based on self-reported height and weight .
	manualset3
134164	6	406350	13	NULL	NULL	0	NULL	non-Veterans 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from national telephone surveys suggest higher prevalence of overweight among Veterans compared with demographically similar non-Veterans , based on self-reported height and weight .
	manualset3
134165	7	406350	13	NULL	NULL	0	NULL	height	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from national telephone surveys suggest higher prevalence of overweight among Veterans compared with demographically similar non-Veterans , based on self-reported height and weight .
	manualset3
134166	8	406350	13	NULL	NULL	0	NULL	weight	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from national telephone surveys suggest higher prevalence of overweight among Veterans compared with demographically similar non-Veterans , based on self-reported height and weight .
	manualset3
134167	1	406351	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from the 2001-2002 study also indicate that the presence of Dermacentor reticulatus adult females is significantly less frequent among infected than non-infected dogs ( OR = 0.44 ; 95 % CI : 0.21-0 .92 ) .
	manualset3
134168	2	406351	13	NULL	NULL	0	NULL	2001-2002 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from the 2001-2002 study also indicate that the presence of Dermacentor reticulatus adult females is significantly less frequent among infected than non-infected dogs ( OR = 0.44 ; 95 % CI : 0.21-0 .92 ) .
	manualset3
134169	3	406351	13	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from the 2001-2002 study also indicate that the presence of Dermacentor reticulatus adult females is significantly less frequent among infected than non-infected dogs ( OR = 0.44 ; 95 % CI : 0.21-0 .92 ) .
	manualset3
134170	4	406351	13	NULL	NULL	0	NULL	 Dermacentor reticulatus adult females	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from the 2001-2002 study also indicate that the presence of Dermacentor reticulatus adult females is significantly less frequent among infected than non-infected dogs ( OR = 0.44 ; 95 % CI : 0.21-0 .92 ) .
	manualset3
134171	5	406351	13	NULL	NULL	NULL	NULL	dogs 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Results from the 2001-2002 study also indicate that the presence of Dermacentor reticulatus adult females is significantly less frequent among infected than non-infected dogs ( OR = 0.44 ; 95 % CI : 0.21-0 .92 ) .
	manualset3
134172	6	406351	13	NULL	NULL	0	NULL	R = 0.44	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from the 2001-2002 study also indicate that the presence of Dermacentor reticulatus adult females is significantly less frequent among infected than non-infected dogs ( OR = 0.44 ; 95 % CI : 0.21-0 .92 ) .
	manualset3
134173	7	406351	13	NULL	NULL	0	NULL	95 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from the 2001-2002 study also indicate that the presence of Dermacentor reticulatus adult females is significantly less frequent among infected than non-infected dogs ( OR = 0.44 ; 95 % CI : 0.21-0 .92 ) .
	manualset3
134174	8	406351	13	NULL	NULL	0	NULL	CI : 0.21-0 .92	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from the 2001-2002 study also indicate that the presence of Dermacentor reticulatus adult females is significantly less frequent among infected than non-infected dogs ( OR = 0.44 ; 95 % CI : 0.21-0 .92 ) .
	manualset3
134175	1	406352	13	NULL	NULL	0	NULL	Results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from the randomized trial conducted by the Health Insurance Plan ( HIP ) to determine the efficacy of breast cancer screening with mammography and palpation are reported for longer periods than previously available .
	manualset3
134177	2	406352	13	NULL	NULL	0	NULL	randomized trial 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from the randomized trial conducted by the Health Insurance Plan ( HIP ) to determine the efficacy of breast cancer screening with mammography and palpation are reported for longer periods than previously available .
	manualset3
134179	3	406352	13	NULL	NULL	0	NULL	Health Insurance Plan ( HIP )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from the randomized trial conducted by the Health Insurance Plan ( HIP ) to determine the efficacy of breast cancer screening with mammography and palpation are reported for longer periods than previously available .
	manualset3
134180	4	406352	13	NULL	NULL	0	NULL	efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from the randomized trial conducted by the Health Insurance Plan ( HIP ) to determine the efficacy of breast cancer screening with mammography and palpation are reported for longer periods than previously available .
	manualset3
134181	5	406352	13	NULL	NULL	0	NULL	breast cancer screening	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from the randomized trial conducted by the Health Insurance Plan ( HIP ) to determine the efficacy of breast cancer screening with mammography and palpation are reported for longer periods than previously available .
	manualset3
134182	6	406352	13	NULL	NULL	0	NULL	mammography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from the randomized trial conducted by the Health Insurance Plan ( HIP ) to determine the efficacy of breast cancer screening with mammography and palpation are reported for longer periods than previously available .
	manualset3
134183	7	406352	13	NULL	NULL	0	NULL	palpation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from the randomized trial conducted by the Health Insurance Plan ( HIP ) to determine the efficacy of breast cancer screening with mammography and palpation are reported for longer periods than previously available .
	manualset3
134184	8	406352	13	NULL	NULL	0	NULL	periods	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from the randomized trial conducted by the Health Insurance Plan ( HIP ) to determine the efficacy of breast cancer screening with mammography and palpation are reported for longer periods than previously available .
	manualset3
134185	1	406353	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from the various analyses are largely concordant with each other as well as with prior analyses of partial mitochondrial large-subunit rDNA ( mtLSU rDNA ) .
	manualset3
134186	2	406353	13	NULL	NULL	0	NULL	various analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from the various analyses are largely concordant with each other as well as with prior analyses of partial mitochondrial large-subunit rDNA ( mtLSU rDNA ) .
	manualset3
134187	3	406353	13	NULL	NULL	0	NULL	prior analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from the various analyses are largely concordant with each other as well as with prior analyses of partial mitochondrial large-subunit rDNA ( mtLSU rDNA ) .
	manualset3
134188	4	406353	13	NULL	NULL	0	NULL	partial mitochondrial large-subunit rDNA ( mtLSU rDNA ) 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from the various analyses are largely concordant with each other as well as with prior analyses of partial mitochondrial large-subunit rDNA ( mtLSU rDNA ) .
	manualset3
134189	1	406354	13	NULL	NULL	0	NULL	Results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from these studies also add to the problems that confront theories positing that the BG selects movement , inhibits unwanted motor responses , corrects errors on-line , or stores and produces well-learned motor skills .
	manualset3
134190	2	406354	13	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from these studies also add to the problems that confront theories positing that the BG selects movement , inhibits unwanted motor responses , corrects errors on-line , or stores and produces well-learned motor skills .
	manualset3
134191	3	406354	13	NULL	NULL	0	NULL	problems	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from these studies also add to the problems that confront theories positing that the BG selects movement , inhibits unwanted motor responses , corrects errors on-line , or stores and produces well-learned motor skills .
	manualset3
134192	4	406354	13	NULL	NULL	0	NULL	theories	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from these studies also add to the problems that confront theories positing that the BG selects movement , inhibits unwanted motor responses , corrects errors on-line , or stores and produces well-learned motor skills .
	manualset3
134193	5	406354	13	NULL	NULL	0	NULL	BG 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from these studies also add to the problems that confront theories positing that the BG selects movement , inhibits unwanted motor responses , corrects errors on-line , or stores and produces well-learned motor skills .
	manualset3
134194	6	406354	13	NULL	NULL	0	NULL	movement	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from these studies also add to the problems that confront theories positing that the BG selects movement , inhibits unwanted motor responses , corrects errors on-line , or stores and produces well-learned motor skills .
	manualset3
134195	7	406354	13	NULL	NULL	0	NULL	motor responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from these studies also add to the problems that confront theories positing that the BG selects movement , inhibits unwanted motor responses , corrects errors on-line , or stores and produces well-learned motor skills .
	manualset3
134196	8	406354	13	NULL	NULL	NULL	NULL	errors	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Results from these studies also add to the problems that confront theories positing that the BG selects movement , inhibits unwanted motor responses , corrects errors on-line , or stores and produces well-learned motor skills .
	manualset3
134198	10	406354	13	NULL	NULL	0	NULL	motor skills	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from these studies also add to the problems that confront theories positing that the BG selects movement , inhibits unwanted motor responses , corrects errors on-line , or stores and produces well-learned motor skills .
	manualset3
134199	1	406355	13	NULL	NULL	0	NULL	Results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from these studies suggest that mutations in RNASEL predispose men to an increased incidence of prostate cancer , which in some cases reflect more aggressive disease and/or decreased age of onset compared with non-RNASEL linked cases .
	manualset3
134200	2	406355	13	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from these studies suggest that mutations in RNASEL predispose men to an increased incidence of prostate cancer , which in some cases reflect more aggressive disease and/or decreased age of onset compared with non-RNASEL linked cases .
	manualset3
134201	3	406355	13	NULL	NULL	0	NULL	mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from these studies suggest that mutations in RNASEL predispose men to an increased incidence of prostate cancer , which in some cases reflect more aggressive disease and/or decreased age of onset compared with non-RNASEL linked cases .
	manualset3
134202	4	406355	13	NULL	NULL	0	NULL	RNASEL	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from these studies suggest that mutations in RNASEL predispose men to an increased incidence of prostate cancer , which in some cases reflect more aggressive disease and/or decreased age of onset compared with non-RNASEL linked cases .
	manualset3
134203	5	406355	13	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from these studies suggest that mutations in RNASEL predispose men to an increased incidence of prostate cancer , which in some cases reflect more aggressive disease and/or decreased age of onset compared with non-RNASEL linked cases .
	manualset3
134204	6	406355	13	NULL	NULL	0	NULL	incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from these studies suggest that mutations in RNASEL predispose men to an increased incidence of prostate cancer , which in some cases reflect more aggressive disease and/or decreased age of onset compared with non-RNASEL linked cases .
	manualset3
134205	7	406355	13	NULL	NULL	0	NULL	prostate cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from these studies suggest that mutations in RNASEL predispose men to an increased incidence of prostate cancer , which in some cases reflect more aggressive disease and/or decreased age of onset compared with non-RNASEL linked cases .
	manualset3
134206	8	406355	13	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from these studies suggest that mutations in RNASEL predispose men to an increased incidence of prostate cancer , which in some cases reflect more aggressive disease and/or decreased age of onset compared with non-RNASEL linked cases .
	manualset3
134207	9	406355	13	NULL	NULL	0	NULL	aggressive disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from these studies suggest that mutations in RNASEL predispose men to an increased incidence of prostate cancer , which in some cases reflect more aggressive disease and/or decreased age of onset compared with non-RNASEL linked cases .
	manualset3
134208	10	406355	13	NULL	NULL	0	NULL	age of onset	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from these studies suggest that mutations in RNASEL predispose men to an increased incidence of prostate cancer , which in some cases reflect more aggressive disease and/or decreased age of onset compared with non-RNASEL linked cases .
	manualset3
134209	11	406355	13	NULL	NULL	0	NULL	non-RNASEL linked cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from these studies suggest that mutations in RNASEL predispose men to an increased incidence of prostate cancer , which in some cases reflect more aggressive disease and/or decreased age of onset compared with non-RNASEL linked cases .
	manualset3
134210	1	406356	13	NULL	NULL	0	NULL	Results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from these three groups showed high coherence of the sound signals and that the discrepancy between both hips was smallest in the frequency range of 200-315 Hz .
	manualset3
134211	2	406356	13	NULL	NULL	0	NULL	three groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from these three groups showed high coherence of the sound signals and that the discrepancy between both hips was smallest in the frequency range of 200-315 Hz .
	manualset3
134212	3	406356	13	NULL	NULL	0	NULL	coherence 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from these three groups showed high coherence of the sound signals and that the discrepancy between both hips was smallest in the frequency range of 200-315 Hz .
	manualset3
134213	4	406356	13	NULL	NULL	0	NULL	sound signals	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from these three groups showed high coherence of the sound signals and that the discrepancy between both hips was smallest in the frequency range of 200-315 Hz .
	manualset3
134214	5	406356	13	NULL	NULL	0	NULL	discrepancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from these three groups showed high coherence of the sound signals and that the discrepancy between both hips was smallest in the frequency range of 200-315 Hz .
	manualset3
134215	6	406356	13	NULL	NULL	0	NULL	both hips	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from these three groups showed high coherence of the sound signals and that the discrepancy between both hips was smallest in the frequency range of 200-315 Hz .
	manualset3
134216	7	406356	13	NULL	NULL	0	NULL	frequency range 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from these three groups showed high coherence of the sound signals and that the discrepancy between both hips was smallest in the frequency range of 200-315 Hz .
	manualset3
134217	8	406356	13	NULL	NULL	0	NULL	200-315 Hz	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results from these three groups showed high coherence of the sound signals and that the discrepancy between both hips was smallest in the frequency range of 200-315 Hz .
	manualset3
134218	1	406357	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results illustrate how intervention that focuses on enabling children to choose their own functional goals in the area of physical activity has important implications for enabling participation and building the social networks of children with DCD .
	manualset3
134219	2	406357	13	NULL	NULL	0	NULL	intervention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results illustrate how intervention that focuses on enabling children to choose their own functional goals in the area of physical activity has important implications for enabling participation and building the social networks of children with DCD .
	manualset3
134220	3	406357	13	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results illustrate how intervention that focuses on enabling children to choose their own functional goals in the area of physical activity has important implications for enabling participation and building the social networks of children with DCD .
	manualset3
134221	4	406357	13	NULL	NULL	0	NULL	functional goals	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results illustrate how intervention that focuses on enabling children to choose their own functional goals in the area of physical activity has important implications for enabling participation and building the social networks of children with DCD .
	manualset3
134222	5	406357	13	NULL	NULL	0	NULL	area of physical activity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results illustrate how intervention that focuses on enabling children to choose their own functional goals in the area of physical activity has important implications for enabling participation and building the social networks of children with DCD .
	manualset3
134223	6	406357	13	NULL	NULL	0	NULL	implications 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results illustrate how intervention that focuses on enabling children to choose their own functional goals in the area of physical activity has important implications for enabling participation and building the social networks of children with DCD .
	manualset3
134224	7	406357	13	NULL	NULL	0	NULL	participation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results illustrate how intervention that focuses on enabling children to choose their own functional goals in the area of physical activity has important implications for enabling participation and building the social networks of children with DCD .
	manualset3
134225	8	406357	13	NULL	NULL	0	NULL	social networks 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results illustrate how intervention that focuses on enabling children to choose their own functional goals in the area of physical activity has important implications for enabling participation and building the social networks of children with DCD .
	manualset3
134226	9	406357	13	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results illustrate how intervention that focuses on enabling children to choose their own functional goals in the area of physical activity has important implications for enabling participation and building the social networks of children with DCD .
	manualset3
134227	10	406357	13	NULL	NULL	0	NULL	DCD	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results illustrate how intervention that focuses on enabling children to choose their own functional goals in the area of physical activity has important implications for enabling participation and building the social networks of children with DCD .
	manualset3
134228	1	406358	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicate that military personnel have adequate health literacy skills although variations were noted on the basis of health training and race/ethnicity .
	manualset3
134229	2	406358	13	NULL	NULL	0	NULL	military personnel 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicate that military personnel have adequate health literacy skills although variations were noted on the basis of health training and race/ethnicity .
	manualset3
134230	3	406358	13	NULL	NULL	0	NULL	health literacy skills	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicate that military personnel have adequate health literacy skills although variations were noted on the basis of health training and race/ethnicity .
	manualset3
134231	4	406358	13	NULL	NULL	0	NULL	variations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicate that military personnel have adequate health literacy skills although variations were noted on the basis of health training and race/ethnicity .
	manualset3
134232	5	406358	13	NULL	NULL	0	NULL	basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicate that military personnel have adequate health literacy skills although variations were noted on the basis of health training and race/ethnicity .
	manualset3
134233	6	406358	13	NULL	NULL	0	NULL	health training 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicate that military personnel have adequate health literacy skills although variations were noted on the basis of health training and race/ethnicity .
	manualset3
134234	7	406358	13	NULL	NULL	0	NULL	race/ethnicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicate that military personnel have adequate health literacy skills although variations were noted on the basis of health training and race/ethnicity .
	manualset3
134235	1	406359	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicate that the absorption cross sections of fractal soot clusters can be significantly larger in the mid-IR wavelengths than what is predicted for Rayleigh-limit spheres that have the same total volume .
	manualset3
134236	2	406359	13	NULL	NULL	0	NULL	absorption cross sections	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicate that the absorption cross sections of fractal soot clusters can be significantly larger in the mid-IR wavelengths than what is predicted for Rayleigh-limit spheres that have the same total volume .
	manualset3
134237	3	406359	13	NULL	NULL	0	NULL	fractal soot clusters	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicate that the absorption cross sections of fractal soot clusters can be significantly larger in the mid-IR wavelengths than what is predicted for Rayleigh-limit spheres that have the same total volume .
	manualset3
134238	4	406359	13	NULL	NULL	0	NULL	mid-IR wavelengths	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicate that the absorption cross sections of fractal soot clusters can be significantly larger in the mid-IR wavelengths than what is predicted for Rayleigh-limit spheres that have the same total volume .
	manualset3
134239	5	406359	13	NULL	NULL	0	NULL	Rayleigh-limit spheres	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicate that the absorption cross sections of fractal soot clusters can be significantly larger in the mid-IR wavelengths than what is predicted for Rayleigh-limit spheres that have the same total volume .
	manualset3
134240	6	406359	13	NULL	NULL	0	NULL	total volume	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicate that the absorption cross sections of fractal soot clusters can be significantly larger in the mid-IR wavelengths than what is predicted for Rayleigh-limit spheres that have the same total volume .
	manualset3
134241	1	406360	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that PUF enhanced PHA - , Con A - , and PWM-induced lymphocyte mitogenesis by 222 % , 207 % , and 261 % , respectively , as compared to control .
	manualset3
134242	2	406360	13	NULL	NULL	0	NULL	PUF	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that PUF enhanced PHA - , Con A - , and PWM-induced lymphocyte mitogenesis by 222 % , 207 % , and 261 % , respectively , as compared to control .
	manualset3
134243	3	406360	13	NULL	NULL	0	NULL	PHA-induced lymphocyte mitogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that PUF enhanced PHA - , Con A - , and PWM-induced lymphocyte mitogenesis by 222 % , 207 % , and 261 % , respectively , as compared to control .
	manualset3
134244	4	406360	13	NULL	NULL	0	NULL	PWM-induced lymphocyte mitogenesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that PUF enhanced PHA - , Con A - , and PWM-induced lymphocyte mitogenesis by 222 % , 207 % , and 261 % , respectively , as compared to control .
	manualset3
134245	5	406360	13	NULL	NULL	0	NULL	Con A -induced lymphocyte mitogenesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that PUF enhanced PHA - , Con A - , and PWM-induced lymphocyte mitogenesis by 222 % , 207 % , and 261 % , respectively , as compared to control .
	manualset3
134246	6	406360	13	NULL	NULL	0	NULL	222 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that PUF enhanced PHA - , Con A - , and PWM-induced lymphocyte mitogenesis by 222 % , 207 % , and 261 % , respectively , as compared to control .
	manualset3
134247	7	406360	13	NULL	NULL	0	NULL	207 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that PUF enhanced PHA - , Con A - , and PWM-induced lymphocyte mitogenesis by 222 % , 207 % , and 261 % , respectively , as compared to control .
	manualset3
134248	8	406360	13	NULL	NULL	0	NULL	261 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that PUF enhanced PHA - , Con A - , and PWM-induced lymphocyte mitogenesis by 222 % , 207 % , and 261 % , respectively , as compared to control .
	manualset3
134249	9	406360	13	NULL	NULL	0	NULL	control 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that PUF enhanced PHA - , Con A - , and PWM-induced lymphocyte mitogenesis by 222 % , 207 % , and 261 % , respectively , as compared to control .
	manualset3
134250	1	406361	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that essential oil of E. cardamomum toxic to the bruchid beetle , Callosobruchus maculatus Fabricius ( Coleoptera : Bruchidae ) , the red flour beetle , Tribolium castaneum Herbst ( Coleoptera : Tenebrionidae ) , and the flour moth , Ephestia kuehniella Zeller ( Lepidoptera : Pyralidae ) .
	manualset3
134251	2	406361	13	NULL	NULL	0	NULL	essential oil	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that essential oil of E. cardamomum toxic to the bruchid beetle , Callosobruchus maculatus Fabricius ( Coleoptera : Bruchidae ) , the red flour beetle , Tribolium castaneum Herbst ( Coleoptera : Tenebrionidae ) , and the flour moth , Ephestia kuehniella Zeller ( Lepidoptera : Pyralidae ) .
	manualset3
134252	3	406361	13	NULL	NULL	0	NULL	E. cardamomum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that essential oil of E. cardamomum toxic to the bruchid beetle , Callosobruchus maculatus Fabricius ( Coleoptera : Bruchidae ) , the red flour beetle , Tribolium castaneum Herbst ( Coleoptera : Tenebrionidae ) , and the flour moth , Ephestia kuehniella Zeller ( Lepidoptera : Pyralidae ) .
	manualset3
134253	4	406361	13	NULL	NULL	0	NULL	bruchid beetle 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that essential oil of E. cardamomum toxic to the bruchid beetle , Callosobruchus maculatus Fabricius ( Coleoptera : Bruchidae ) , the red flour beetle , Tribolium castaneum Herbst ( Coleoptera : Tenebrionidae ) , and the flour moth , Ephestia kuehniella Zeller ( Lepidoptera : Pyralidae ) .
	manualset3
134254	5	406361	13	NULL	NULL	0	NULL	Callosobruchus maculatus Fabricius	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that essential oil of E. cardamomum toxic to the bruchid beetle , Callosobruchus maculatus Fabricius ( Coleoptera : Bruchidae ) , the red flour beetle , Tribolium castaneum Herbst ( Coleoptera : Tenebrionidae ) , and the flour moth , Ephestia kuehniella Zeller ( Lepidoptera : Pyralidae ) .
	manualset3
134255	6	406361	13	NULL	NULL	0	NULL	 Coleoptera : Bruchidae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that essential oil of E. cardamomum toxic to the bruchid beetle , Callosobruchus maculatus Fabricius ( Coleoptera : Bruchidae ) , the red flour beetle , Tribolium castaneum Herbst ( Coleoptera : Tenebrionidae ) , and the flour moth , Ephestia kuehniella Zeller ( Lepidoptera : Pyralidae ) .
	manualset3
134256	7	406361	13	NULL	NULL	0	NULL	red flour beetle	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that essential oil of E. cardamomum toxic to the bruchid beetle , Callosobruchus maculatus Fabricius ( Coleoptera : Bruchidae ) , the red flour beetle , Tribolium castaneum Herbst ( Coleoptera : Tenebrionidae ) , and the flour moth , Ephestia kuehniella Zeller ( Lepidoptera : Pyralidae ) .
	manualset3
134257	8	406361	13	NULL	NULL	0	NULL	Tribolium castaneum Herbst	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that essential oil of E. cardamomum toxic to the bruchid beetle , Callosobruchus maculatus Fabricius ( Coleoptera : Bruchidae ) , the red flour beetle , Tribolium castaneum Herbst ( Coleoptera : Tenebrionidae ) , and the flour moth , Ephestia kuehniella Zeller ( Lepidoptera : Pyralidae ) .
	manualset3
134258	9	406361	13	NULL	NULL	0	NULL	Coleoptera : Tenebrionidae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that essential oil of E. cardamomum toxic to the bruchid beetle , Callosobruchus maculatus Fabricius ( Coleoptera : Bruchidae ) , the red flour beetle , Tribolium castaneum Herbst ( Coleoptera : Tenebrionidae ) , and the flour moth , Ephestia kuehniella Zeller ( Lepidoptera : Pyralidae ) .
	manualset3
134259	10	406361	13	NULL	NULL	0	NULL	flour moth	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that essential oil of E. cardamomum toxic to the bruchid beetle , Callosobruchus maculatus Fabricius ( Coleoptera : Bruchidae ) , the red flour beetle , Tribolium castaneum Herbst ( Coleoptera : Tenebrionidae ) , and the flour moth , Ephestia kuehniella Zeller ( Lepidoptera : Pyralidae ) .
	manualset3
134260	11	406361	13	NULL	NULL	0	NULL	Ephestia kuehniella Zeller	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that essential oil of E. cardamomum toxic to the bruchid beetle , Callosobruchus maculatus Fabricius ( Coleoptera : Bruchidae ) , the red flour beetle , Tribolium castaneum Herbst ( Coleoptera : Tenebrionidae ) , and the flour moth , Ephestia kuehniella Zeller ( Lepidoptera : Pyralidae ) .
	manualset3
134261	12	406361	13	NULL	NULL	0	NULL	Lepidoptera : Pyralidae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that essential oil of E. cardamomum toxic to the bruchid beetle , Callosobruchus maculatus Fabricius ( Coleoptera : Bruchidae ) , the red flour beetle , Tribolium castaneum Herbst ( Coleoptera : Tenebrionidae ) , and the flour moth , Ephestia kuehniella Zeller ( Lepidoptera : Pyralidae ) .
	manualset3
134262	1	406362	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that rumination was sufficient to elevate blood pressure ( systolic and diastolic ) above baseline , that the delay made no difference to the magnitude of the elevation , but that the second rumination seemed to be associated with a smaller response than the first .
	manualset3
134263	2	406362	13	NULL	NULL	0	NULL	rumination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that rumination was sufficient to elevate blood pressure ( systolic and diastolic ) above baseline , that the delay made no difference to the magnitude of the elevation , but that the second rumination seemed to be associated with a smaller response than the first .
	manualset3
134264	3	406362	13	NULL	NULL	0	NULL	blood pressure 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that rumination was sufficient to elevate blood pressure ( systolic and diastolic ) above baseline , that the delay made no difference to the magnitude of the elevation , but that the second rumination seemed to be associated with a smaller response than the first .
	manualset3
134265	4	406362	13	NULL	NULL	0	NULL	baseline	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that rumination was sufficient to elevate blood pressure ( systolic and diastolic ) above baseline , that the delay made no difference to the magnitude of the elevation , but that the second rumination seemed to be associated with a smaller response than the first .
	manualset3
134266	5	406362	13	NULL	NULL	0	NULL	delay	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that rumination was sufficient to elevate blood pressure ( systolic and diastolic ) above baseline , that the delay made no difference to the magnitude of the elevation , but that the second rumination seemed to be associated with a smaller response than the first .
	manualset3
134267	6	406362	13	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that rumination was sufficient to elevate blood pressure ( systolic and diastolic ) above baseline , that the delay made no difference to the magnitude of the elevation , but that the second rumination seemed to be associated with a smaller response than the first .
	manualset3
134268	7	406362	13	NULL	NULL	0	NULL	magnitude	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that rumination was sufficient to elevate blood pressure ( systolic and diastolic ) above baseline , that the delay made no difference to the magnitude of the elevation , but that the second rumination seemed to be associated with a smaller response than the first .
	manualset3
134269	8	406362	13	NULL	NULL	0	NULL	elevation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that rumination was sufficient to elevate blood pressure ( systolic and diastolic ) above baseline , that the delay made no difference to the magnitude of the elevation , but that the second rumination seemed to be associated with a smaller response than the first .
	manualset3
134270	9	406362	13	NULL	NULL	0	NULL	second rumination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that rumination was sufficient to elevate blood pressure ( systolic and diastolic ) above baseline , that the delay made no difference to the magnitude of the elevation , but that the second rumination seemed to be associated with a smaller response than the first .
	manualset3
134271	10	406362	13	NULL	NULL	0	NULL	response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that rumination was sufficient to elevate blood pressure ( systolic and diastolic ) above baseline , that the delay made no difference to the magnitude of the elevation , but that the second rumination seemed to be associated with a smaller response than the first .
	manualset3
134272	1	406363	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the dual layer filtration system recovered 83 + / -14 % of the test bacteria ( Enterococcus fecalis ) and 81 + / -28 % of the test virus ( MS2 coliphage ) on the top and bottom membranes , respectively .
	manualset3
134273	2	406363	13	NULL	NULL	0	NULL	dual layer filtration system 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the dual layer filtration system recovered 83 + / -14 % of the test bacteria ( Enterococcus fecalis ) and 81 + / -28 % of the test virus ( MS2 coliphage ) on the top and bottom membranes , respectively .
	manualset3
134274	3	406363	13	NULL	NULL	0	NULL	83 + / -14 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the dual layer filtration system recovered 83 + / -14 % of the test bacteria ( Enterococcus fecalis ) and 81 + / -28 % of the test virus ( MS2 coliphage ) on the top and bottom membranes , respectively .
	manualset3
134275	4	406363	13	NULL	NULL	0	NULL	test bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the dual layer filtration system recovered 83 + / -14 % of the test bacteria ( Enterococcus fecalis ) and 81 + / -28 % of the test virus ( MS2 coliphage ) on the top and bottom membranes , respectively .
	manualset3
134276	5	406363	13	NULL	NULL	0	NULL	Enterococcus fecalis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the dual layer filtration system recovered 83 + / -14 % of the test bacteria ( Enterococcus fecalis ) and 81 + / -28 % of the test virus ( MS2 coliphage ) on the top and bottom membranes , respectively .
	manualset3
134277	6	406363	13	NULL	NULL	0	NULL	81 + / -28 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the dual layer filtration system recovered 83 + / -14 % of the test bacteria ( Enterococcus fecalis ) and 81 + / -28 % of the test virus ( MS2 coliphage ) on the top and bottom membranes , respectively .
	manualset3
134278	7	406363	13	NULL	NULL	0	NULL	test virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the dual layer filtration system recovered 83 + / -14 % of the test bacteria ( Enterococcus fecalis ) and 81 + / -28 % of the test virus ( MS2 coliphage ) on the top and bottom membranes , respectively .
	manualset3
134279	8	406363	13	NULL	NULL	0	NULL	MS2 coliphage	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the dual layer filtration system recovered 83 + / -14 % of the test bacteria ( Enterococcus fecalis ) and 81 + / -28 % of the test virus ( MS2 coliphage ) on the top and bottom membranes , respectively .
	manualset3
134280	9	406363	13	NULL	NULL	0	NULL	top membrane	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the dual layer filtration system recovered 83 + / -14 % of the test bacteria ( Enterococcus fecalis ) and 81 + / -28 % of the test virus ( MS2 coliphage ) on the top and bottom membranes , respectively .
	manualset3
134281	10	406363	13	NULL	NULL	0	NULL	bottom membrane	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the dual layer filtration system recovered 83 + / -14 % of the test bacteria ( Enterococcus fecalis ) and 81 + / -28 % of the test virus ( MS2 coliphage ) on the top and bottom membranes , respectively .
	manualset3
134282	1	406364	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the strain was able to utilize 2 , 6-DTBP , lysine , lactamine , citrate , n-utenedioic acid and malic acid as the sole carbon and energy source , alkalinize acetamide , asparagine , L-histidine , acetate , citrate and propionate , but failed to utilize glucose , D-fructose , D-seminose , D-xylose , serine and phenylalanine as the sole carbon and energy source .
	manualset3
134283	2	406364	13	NULL	NULL	0	NULL	strain 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the strain was able to utilize 2 , 6-DTBP , lysine , lactamine , citrate , n-utenedioic acid and malic acid as the sole carbon and energy source , alkalinize acetamide , asparagine , L-histidine , acetate , citrate and propionate , but failed to utilize glucose , D-fructose , D-seminose , D-xylose , serine and phenylalanine as the sole carbon and energy source .
	manualset3
134284	3	406364	13	NULL	NULL	0	NULL	6-DTBP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the strain was able to utilize 2 , 6-DTBP , lysine , lactamine , citrate , n-utenedioic acid and malic acid as the sole carbon and energy source , alkalinize acetamide , asparagine , L-histidine , acetate , citrate and propionate , but failed to utilize glucose , D-fructose , D-seminose , D-xylose , serine and phenylalanine as the sole carbon and energy source .
	manualset3
134285	4	406364	13	NULL	NULL	0	NULL	lysine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the strain was able to utilize 2 , 6-DTBP , lysine , lactamine , citrate , n-utenedioic acid and malic acid as the sole carbon and energy source , alkalinize acetamide , asparagine , L-histidine , acetate , citrate and propionate , but failed to utilize glucose , D-fructose , D-seminose , D-xylose , serine and phenylalanine as the sole carbon and energy source .
	manualset3
134286	5	406364	13	NULL	NULL	0	NULL	lactamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the strain was able to utilize 2 , 6-DTBP , lysine , lactamine , citrate , n-utenedioic acid and malic acid as the sole carbon and energy source , alkalinize acetamide , asparagine , L-histidine , acetate , citrate and propionate , but failed to utilize glucose , D-fructose , D-seminose , D-xylose , serine and phenylalanine as the sole carbon and energy source .
	manualset3
134287	6	406364	13	NULL	NULL	0	NULL	citrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the strain was able to utilize 2 , 6-DTBP , lysine , lactamine , citrate , n-utenedioic acid and malic acid as the sole carbon and energy source , alkalinize acetamide , asparagine , L-histidine , acetate , citrate and propionate , but failed to utilize glucose , D-fructose , D-seminose , D-xylose , serine and phenylalanine as the sole carbon and energy source .
	manualset3
134288	7	406364	13	NULL	NULL	0	NULL	n-utenedioic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the strain was able to utilize 2 , 6-DTBP , lysine , lactamine , citrate , n-utenedioic acid and malic acid as the sole carbon and energy source , alkalinize acetamide , asparagine , L-histidine , acetate , citrate and propionate , but failed to utilize glucose , D-fructose , D-seminose , D-xylose , serine and phenylalanine as the sole carbon and energy source .
	manualset3
134289	8	406364	13	NULL	NULL	0	NULL	malic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the strain was able to utilize 2 , 6-DTBP , lysine , lactamine , citrate , n-utenedioic acid and malic acid as the sole carbon and energy source , alkalinize acetamide , asparagine , L-histidine , acetate , citrate and propionate , but failed to utilize glucose , D-fructose , D-seminose , D-xylose , serine and phenylalanine as the sole carbon and energy source .
	manualset3
134290	9	406364	13	NULL	NULL	0	NULL	sole carbon source 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the strain was able to utilize 2 , 6-DTBP , lysine , lactamine , citrate , n-utenedioic acid and malic acid as the sole carbon and energy source , alkalinize acetamide , asparagine , L-histidine , acetate , citrate and propionate , but failed to utilize glucose , D-fructose , D-seminose , D-xylose , serine and phenylalanine as the sole carbon and energy source .
	manualset3
134291	10	406364	13	NULL	NULL	0	NULL	energy source	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the strain was able to utilize 2 , 6-DTBP , lysine , lactamine , citrate , n-utenedioic acid and malic acid as the sole carbon and energy source , alkalinize acetamide , asparagine , L-histidine , acetate , citrate and propionate , but failed to utilize glucose , D-fructose , D-seminose , D-xylose , serine and phenylalanine as the sole carbon and energy source .
	manualset3
134292	11	406364	13	NULL	NULL	0	NULL	alkalinize acetamide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the strain was able to utilize 2 , 6-DTBP , lysine , lactamine , citrate , n-utenedioic acid and malic acid as the sole carbon and energy source , alkalinize acetamide , asparagine , L-histidine , acetate , citrate and propionate , but failed to utilize glucose , D-fructose , D-seminose , D-xylose , serine and phenylalanine as the sole carbon and energy source .
	manualset3
134293	12	406364	13	NULL	NULL	0	NULL	asparagine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the strain was able to utilize 2 , 6-DTBP , lysine , lactamine , citrate , n-utenedioic acid and malic acid as the sole carbon and energy source , alkalinize acetamide , asparagine , L-histidine , acetate , citrate and propionate , but failed to utilize glucose , D-fructose , D-seminose , D-xylose , serine and phenylalanine as the sole carbon and energy source .
	manualset3
134294	13	406364	13	NULL	NULL	0	NULL	L-histidine 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the strain was able to utilize 2 , 6-DTBP , lysine , lactamine , citrate , n-utenedioic acid and malic acid as the sole carbon and energy source , alkalinize acetamide , asparagine , L-histidine , acetate , citrate and propionate , but failed to utilize glucose , D-fructose , D-seminose , D-xylose , serine and phenylalanine as the sole carbon and energy source .
	manualset3
134295	14	406364	13	NULL	NULL	0	NULL	acetate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the strain was able to utilize 2 , 6-DTBP , lysine , lactamine , citrate , n-utenedioic acid and malic acid as the sole carbon and energy source , alkalinize acetamide , asparagine , L-histidine , acetate , citrate and propionate , but failed to utilize glucose , D-fructose , D-seminose , D-xylose , serine and phenylalanine as the sole carbon and energy source .
	manualset3
134296	15	406364	13	NULL	NULL	0	NULL	citrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the strain was able to utilize 2 , 6-DTBP , lysine , lactamine , citrate , n-utenedioic acid and malic acid as the sole carbon and energy source , alkalinize acetamide , asparagine , L-histidine , acetate , citrate and propionate , but failed to utilize glucose , D-fructose , D-seminose , D-xylose , serine and phenylalanine as the sole carbon and energy source .
	manualset3
134297	16	406364	13	NULL	NULL	0	NULL	propionate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the strain was able to utilize 2 , 6-DTBP , lysine , lactamine , citrate , n-utenedioic acid and malic acid as the sole carbon and energy source , alkalinize acetamide , asparagine , L-histidine , acetate , citrate and propionate , but failed to utilize glucose , D-fructose , D-seminose , D-xylose , serine and phenylalanine as the sole carbon and energy source .
	manualset3
134298	17	406364	13	NULL	NULL	0	NULL	glucose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the strain was able to utilize 2 , 6-DTBP , lysine , lactamine , citrate , n-utenedioic acid and malic acid as the sole carbon and energy source , alkalinize acetamide , asparagine , L-histidine , acetate , citrate and propionate , but failed to utilize glucose , D-fructose , D-seminose , D-xylose , serine and phenylalanine as the sole carbon and energy source .
	manualset3
134299	18	406364	13	NULL	NULL	0	NULL	D-fructose 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the strain was able to utilize 2 , 6-DTBP , lysine , lactamine , citrate , n-utenedioic acid and malic acid as the sole carbon and energy source , alkalinize acetamide , asparagine , L-histidine , acetate , citrate and propionate , but failed to utilize glucose , D-fructose , D-seminose , D-xylose , serine and phenylalanine as the sole carbon and energy source .
	manualset3
134300	19	406364	13	NULL	NULL	0	NULL	D-seminose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the strain was able to utilize 2 , 6-DTBP , lysine , lactamine , citrate , n-utenedioic acid and malic acid as the sole carbon and energy source , alkalinize acetamide , asparagine , L-histidine , acetate , citrate and propionate , but failed to utilize glucose , D-fructose , D-seminose , D-xylose , serine and phenylalanine as the sole carbon and energy source .
	manualset3
134301	20	406364	13	NULL	NULL	0	NULL	D-xylose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the strain was able to utilize 2 , 6-DTBP , lysine , lactamine , citrate , n-utenedioic acid and malic acid as the sole carbon and energy source , alkalinize acetamide , asparagine , L-histidine , acetate , citrate and propionate , but failed to utilize glucose , D-fructose , D-seminose , D-xylose , serine and phenylalanine as the sole carbon and energy source .
	manualset3
134302	21	406364	13	NULL	NULL	NULL	NULL	serine	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Results indicated that the strain was able to utilize 2 , 6-DTBP , lysine , lactamine , citrate , n-utenedioic acid and malic acid as the sole carbon and energy source , alkalinize acetamide , asparagine , L-histidine , acetate , citrate and propionate , but failed to utilize glucose , D-fructose , D-seminose , D-xylose , serine and phenylalanine as the sole carbon and energy source .
	manualset3
134303	22	406364	13	NULL	NULL	0	NULL	phenylalanine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the strain was able to utilize 2 , 6-DTBP , lysine , lactamine , citrate , n-utenedioic acid and malic acid as the sole carbon and energy source , alkalinize acetamide , asparagine , L-histidine , acetate , citrate and propionate , but failed to utilize glucose , D-fructose , D-seminose , D-xylose , serine and phenylalanine as the sole carbon and energy source .
	manualset3
134304	23	406364	13	NULL	NULL	0	NULL	sole carbon source	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the strain was able to utilize 2 , 6-DTBP , lysine , lactamine , citrate , n-utenedioic acid and malic acid as the sole carbon and energy source , alkalinize acetamide , asparagine , L-histidine , acetate , citrate and propionate , but failed to utilize glucose , D-fructose , D-seminose , D-xylose , serine and phenylalanine as the sole carbon and energy source .
	manualset3
134305	24	406364	13	NULL	NULL	0	NULL	energy source 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that the strain was able to utilize 2 , 6-DTBP , lysine , lactamine , citrate , n-utenedioic acid and malic acid as the sole carbon and energy source , alkalinize acetamide , asparagine , L-histidine , acetate , citrate and propionate , but failed to utilize glucose , D-fructose , D-seminose , D-xylose , serine and phenylalanine as the sole carbon and energy source .
	manualset3
134315	1	406365	13	NULL	NULL	0	NULL	Results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that while overall cognitive impairment increased with advancing disease , the pattern of neuropsychological impairments were not different with respect to laterality of motor symptoms in either experiment .
	manualset3
134316	2	406365	13	NULL	NULL	0	NULL	cognitive impairment 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that while overall cognitive impairment increased with advancing disease , the pattern of neuropsychological impairments were not different with respect to laterality of motor symptoms in either experiment .
	manualset3
134317	3	406365	13	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that while overall cognitive impairment increased with advancing disease , the pattern of neuropsychological impairments were not different with respect to laterality of motor symptoms in either experiment .
	manualset3
134327	4	406365	13	NULL	NULL	0	NULL	pattern	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that while overall cognitive impairment increased with advancing disease , the pattern of neuropsychological impairments were not different with respect to laterality of motor symptoms in either experiment .
	manualset3
134329	5	406365	13	NULL	NULL	0	NULL	neuropsychological impairments	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that while overall cognitive impairment increased with advancing disease , the pattern of neuropsychological impairments were not different with respect to laterality of motor symptoms in either experiment .
	manualset3
134330	6	406365	13	NULL	NULL	0	NULL	respect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that while overall cognitive impairment increased with advancing disease , the pattern of neuropsychological impairments were not different with respect to laterality of motor symptoms in either experiment .
	manualset3
134332	7	406365	13	NULL	NULL	0	NULL	laterality of motor symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that while overall cognitive impairment increased with advancing disease , the pattern of neuropsychological impairments were not different with respect to laterality of motor symptoms in either experiment .
	manualset3
134333	8	406365	13	NULL	NULL	0	NULL	experiment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results indicated that while overall cognitive impairment increased with advancing disease , the pattern of neuropsychological impairments were not different with respect to laterality of motor symptoms in either experiment .
	manualset3
134402	1	406366	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results obtained by physical and chemical treatments suggest that hemagglutinin for Phallusia mamillata and Ascidia malaca may be a protein or a protein-like substance .
	manualset3
134403	2	406366	13	NULL	NULL	0	NULL	physical treatments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results obtained by physical and chemical treatments suggest that hemagglutinin for Phallusia mamillata and Ascidia malaca may be a protein or a protein-like substance .
	manualset3
134404	3	406366	13	NULL	NULL	0	NULL	chemical treatments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results obtained by physical and chemical treatments suggest that hemagglutinin for Phallusia mamillata and Ascidia malaca may be a protein or a protein-like substance .
	manualset3
134405	4	406366	13	NULL	NULL	0	NULL	hemagglutinin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Results obtained by physical and chemical treatments suggest that hemagglutinin for Phallusia mamillata and Ascidia malaca may be a protein or a protein-like substance .
	manualset3
134406	5	406366	13	NULL	NULL	0	NULL	Phallusia mamillata 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Results obtained by physical and chemical treatments suggest that hemagglutinin for Phallusia mamillata and Ascidia malaca may be a protein or a protein-like substance .
	manualset3
134407	6	406366	13	NULL	NULL	0	NULL	Ascidia malaca	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Results obtained by physical and chemical treatments suggest that hemagglutinin for Phallusia mamillata and Ascidia malaca may be a protein or a protein-like substance .
	manualset3
134408	7	406366	13	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Results obtained by physical and chemical treatments suggest that hemagglutinin for Phallusia mamillata and Ascidia malaca may be a protein or a protein-like substance .
	manualset3
134409	8	406366	13	NULL	NULL	0	NULL	protein-like substance	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Results obtained by physical and chemical treatments suggest that hemagglutinin for Phallusia mamillata and Ascidia malaca may be a protein or a protein-like substance .
	manualset3
134410	1	406367	13	NULL	NULL	0	NULL	Results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results obtained showed that AlCl3 significantly ( p & lt ; 0.05 ) induced free radicals ( thiobarbituric acid-reactive substances ) and decreased the activity of glutathione S-transferase ( GST ) and the levels of sulphydryl groups ( SH groups ) in rat plasma , liver , brain , testes and kidney .
	manualset3
134411	2	406367	13	NULL	NULL	0	NULL	AlCl3	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results obtained showed that AlCl3 significantly ( p & lt ; 0.05 ) induced free radicals ( thiobarbituric acid-reactive substances ) and decreased the activity of glutathione S-transferase ( GST ) and the levels of sulphydryl groups ( SH groups ) in rat plasma , liver , brain , testes and kidney .
	manualset3
134412	3	406367	13	NULL	NULL	0	NULL	p & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results obtained showed that AlCl3 significantly ( p & lt ; 0.05 ) induced free radicals ( thiobarbituric acid-reactive substances ) and decreased the activity of glutathione S-transferase ( GST ) and the levels of sulphydryl groups ( SH groups ) in rat plasma , liver , brain , testes and kidney .
	manualset3
134413	4	406367	13	NULL	NULL	0	NULL	free radicals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results obtained showed that AlCl3 significantly ( p & lt ; 0.05 ) induced free radicals ( thiobarbituric acid-reactive substances ) and decreased the activity of glutathione S-transferase ( GST ) and the levels of sulphydryl groups ( SH groups ) in rat plasma , liver , brain , testes and kidney .
	manualset3
134414	5	406367	13	NULL	NULL	0	NULL	thiobarbituric acid-reactive substances	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results obtained showed that AlCl3 significantly ( p & lt ; 0.05 ) induced free radicals ( thiobarbituric acid-reactive substances ) and decreased the activity of glutathione S-transferase ( GST ) and the levels of sulphydryl groups ( SH groups ) in rat plasma , liver , brain , testes and kidney .
	manualset3
134415	6	406367	13	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results obtained showed that AlCl3 significantly ( p & lt ; 0.05 ) induced free radicals ( thiobarbituric acid-reactive substances ) and decreased the activity of glutathione S-transferase ( GST ) and the levels of sulphydryl groups ( SH groups ) in rat plasma , liver , brain , testes and kidney .
	manualset3
134416	7	406367	13	NULL	NULL	0	NULL	glutathione S-transferase ( GST ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Results obtained showed that AlCl3 significantly ( p & lt ; 0.05 ) induced free radicals ( thiobarbituric acid-reactive substances ) and decreased the activity of glutathione S-transferase ( GST ) and the levels of sulphydryl groups ( SH groups ) in rat plasma , liver , brain , testes and kidney .
	manualset3
134417	8	406367	13	NULL	NULL	0	NULL	levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results obtained showed that AlCl3 significantly ( p & lt ; 0.05 ) induced free radicals ( thiobarbituric acid-reactive substances ) and decreased the activity of glutathione S-transferase ( GST ) and the levels of sulphydryl groups ( SH groups ) in rat plasma , liver , brain , testes and kidney .
	manualset3
134418	9	406367	13	NULL	NULL	0	NULL	sulphydryl groups ( SH groups )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results obtained showed that AlCl3 significantly ( p & lt ; 0.05 ) induced free radicals ( thiobarbituric acid-reactive substances ) and decreased the activity of glutathione S-transferase ( GST ) and the levels of sulphydryl groups ( SH groups ) in rat plasma , liver , brain , testes and kidney .
	manualset3
134419	10	406367	13	NULL	NULL	NULL	NULL	rat plasma	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Results obtained showed that AlCl3 significantly ( p & lt ; 0.05 ) induced free radicals ( thiobarbituric acid-reactive substances ) and decreased the activity of glutathione S-transferase ( GST ) and the levels of sulphydryl groups ( SH groups ) in rat plasma , liver , brain , testes and kidney .
	manualset3
134420	11	406367	13	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Results obtained showed that AlCl3 significantly ( p & lt ; 0.05 ) induced free radicals ( thiobarbituric acid-reactive substances ) and decreased the activity of glutathione S-transferase ( GST ) and the levels of sulphydryl groups ( SH groups ) in rat plasma , liver , brain , testes and kidney .
	manualset3
134421	12	406367	13	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Results obtained showed that AlCl3 significantly ( p & lt ; 0.05 ) induced free radicals ( thiobarbituric acid-reactive substances ) and decreased the activity of glutathione S-transferase ( GST ) and the levels of sulphydryl groups ( SH groups ) in rat plasma , liver , brain , testes and kidney .
	manualset3
134422	13	406367	13	NULL	NULL	0	NULL	testes 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Results obtained showed that AlCl3 significantly ( p & lt ; 0.05 ) induced free radicals ( thiobarbituric acid-reactive substances ) and decreased the activity of glutathione S-transferase ( GST ) and the levels of sulphydryl groups ( SH groups ) in rat plasma , liver , brain , testes and kidney .
	manualset3
134423	14	406367	13	NULL	NULL	0	NULL	kidney 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Results obtained showed that AlCl3 significantly ( p & lt ; 0.05 ) induced free radicals ( thiobarbituric acid-reactive substances ) and decreased the activity of glutathione S-transferase ( GST ) and the levels of sulphydryl groups ( SH groups ) in rat plasma , liver , brain , testes and kidney .
	manualset3
134424	1	406368	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of LVM ( 221 + / - 37.9 , g ) were higher than figures reported for others groups .
	manualset3
134425	2	406368	13	NULL	NULL	0	NULL	LVM	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of LVM ( 221 + / - 37.9 , g ) were higher than figures reported for others groups .
	manualset3
134426	3	406368	13	NULL	NULL	0	NULL	221 + / - 37.9 , g	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of LVM ( 221 + / - 37.9 , g ) were higher than figures reported for others groups .
	manualset3
134427	4	406368	13	NULL	NULL	0	NULL	figures	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of LVM ( 221 + / - 37.9 , g ) were higher than figures reported for others groups .
	manualset3
134428	5	406368	13	NULL	NULL	0	NULL	groups 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of LVM ( 221 + / - 37.9 , g ) were higher than figures reported for others groups .
	manualset3
134429	1	406369	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of a 10 min flash distillation and 10 min IC determination compare favorably with the results from the conventional Monier-Williams method for total sulfite in a variety of food matrices .
	manualset3
134430	2	406369	13	NULL	NULL	0	NULL	10 min flash distillation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of a 10 min flash distillation and 10 min IC determination compare favorably with the results from the conventional Monier-Williams method for total sulfite in a variety of food matrices .
	manualset3
134431	3	406369	13	NULL	NULL	0	NULL	10 min IC determination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of a 10 min flash distillation and 10 min IC determination compare favorably with the results from the conventional Monier-Williams method for total sulfite in a variety of food matrices .
	manualset3
134432	4	406369	13	NULL	NULL	0	NULL	compare	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of a 10 min flash distillation and 10 min IC determination compare favorably with the results from the conventional Monier-Williams method for total sulfite in a variety of food matrices .
	manualset3
134433	5	406369	13	NULL	NULL	0	NULL	results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of a 10 min flash distillation and 10 min IC determination compare favorably with the results from the conventional Monier-Williams method for total sulfite in a variety of food matrices .
	manualset3
134434	6	406369	13	NULL	NULL	0	NULL	conventional Monier-Williams method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of a 10 min flash distillation and 10 min IC determination compare favorably with the results from the conventional Monier-Williams method for total sulfite in a variety of food matrices .
	manualset3
134435	7	406369	13	NULL	NULL	0	NULL	total sulfite	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of a 10 min flash distillation and 10 min IC determination compare favorably with the results from the conventional Monier-Williams method for total sulfite in a variety of food matrices .
	manualset3
134436	8	406369	13	NULL	NULL	NULL	NULL	variety of food matrices	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Results of a 10 min flash distillation and 10 min IC determination compare favorably with the results from the conventional Monier-Williams method for total sulfite in a variety of food matrices .
	manualset3
134437	1	406370	13	NULL	NULL	0	NULL	Results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of a year 's prospective study of prolonged laryngo-tracheal intubation with assisted ventilation ) .
	manualset3
134438	2	406370	13	NULL	NULL	0	NULL	year 's	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of a year 's prospective study of prolonged laryngo-tracheal intubation with assisted ventilation ) .
	manualset3
134439	3	406370	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of a year 's prospective study of prolonged laryngo-tracheal intubation with assisted ventilation ) .
	manualset3
134440	4	406370	13	NULL	NULL	0	NULL	laryngo-tracheal intubation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of a year 's prospective study of prolonged laryngo-tracheal intubation with assisted ventilation ) .
	manualset3
134441	5	406370	13	NULL	NULL	0	NULL	ventilation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of a year 's prospective study of prolonged laryngo-tracheal intubation with assisted ventilation ) .
	manualset3
134442	1	406371	13	NULL	NULL	0	NULL	Results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of both in vivo and in vitro experimental studies indicate that signaling pathways related to autophagy might become a target of new neuroprotective strategies .
	manualset3
134443	2	406371	13	NULL	NULL	0	NULL	experimental studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of both in vivo and in vitro experimental studies indicate that signaling pathways related to autophagy might become a target of new neuroprotective strategies .
	manualset3
134444	3	406371	13	NULL	NULL	0	NULL	signaling pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of both in vivo and in vitro experimental studies indicate that signaling pathways related to autophagy might become a target of new neuroprotective strategies .
	manualset3
134445	4	406371	13	NULL	NULL	0	NULL	autophagy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of both in vivo and in vitro experimental studies indicate that signaling pathways related to autophagy might become a target of new neuroprotective strategies .
	manualset3
134446	5	406371	13	NULL	NULL	0	NULL	target 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of both in vivo and in vitro experimental studies indicate that signaling pathways related to autophagy might become a target of new neuroprotective strategies .
	manualset3
134447	6	406371	13	NULL	NULL	NULL	NULL	new neuroprotective strategies	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Results of both in vivo and in vitro experimental studies indicate that signaling pathways related to autophagy might become a target of new neuroprotective strategies .
	manualset3
134448	1	406372	13	NULL	NULL	0	NULL	negative correlation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A negative correlation between societal suicide rates and social integration has been reported using data within individual countries ; however , this has rarely been examined cross-nationally .
	manualset3
134449	2	406372	13	NULL	NULL	0	NULL	societal suicide rates	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A negative correlation between societal suicide rates and social integration has been reported using data within individual countries ; however , this has rarely been examined cross-nationally .
	manualset3
134450	3	406372	13	NULL	NULL	0	NULL	social integration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A negative correlation between societal suicide rates and social integration has been reported using data within individual countries ; however , this has rarely been examined cross-nationally .
	manualset3
134451	4	406372	13	NULL	NULL	0	NULL	data	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A negative correlation between societal suicide rates and social integration has been reported using data within individual countries ; however , this has rarely been examined cross-nationally .
	manualset3
134452	5	406372	13	NULL	NULL	0	NULL	countries 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A negative correlation between societal suicide rates and social integration has been reported using data within individual countries ; however , this has rarely been examined cross-nationally .
	manualset3
134453	1	406373	13	NULL	NULL	0	NULL	Results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of follow-up of human contacts of bovine tuberculosis in cattle during 1993-7 in North Staffordshire .
	manualset3
134454	2	406373	13	NULL	NULL	0	NULL	follow-up	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of follow-up of human contacts of bovine tuberculosis in cattle during 1993-7 in North Staffordshire .
	manualset3
134455	3	406373	13	NULL	NULL	0	NULL	human contacts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of follow-up of human contacts of bovine tuberculosis in cattle during 1993-7 in North Staffordshire .
	manualset3
134456	4	406373	13	NULL	NULL	0	NULL	bovine tuberculosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of follow-up of human contacts of bovine tuberculosis in cattle during 1993-7 in North Staffordshire .
	manualset3
134457	5	406373	13	NULL	NULL	0	NULL	cattle 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of follow-up of human contacts of bovine tuberculosis in cattle during 1993-7 in North Staffordshire .
	manualset3
134458	6	406373	13	NULL	NULL	0	NULL	1993-7	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of follow-up of human contacts of bovine tuberculosis in cattle during 1993-7 in North Staffordshire .
	manualset3
134459	7	406373	13	NULL	NULL	0	NULL	North Staffordshire	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of follow-up of human contacts of bovine tuberculosis in cattle during 1993-7 in North Staffordshire .
	manualset3
134460	1	406374	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of relative standard deviations did not exceed 1.6 % , indicating that the proposed methods having good repeatability and reproducibility .
	manualset3
134461	2	406374	13	NULL	NULL	0	NULL	relative standard deviations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of relative standard deviations did not exceed 1.6 % , indicating that the proposed methods having good repeatability and reproducibility .
	manualset3
134462	3	406374	13	NULL	NULL	0	NULL	1.6 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of relative standard deviations did not exceed 1.6 % , indicating that the proposed methods having good repeatability and reproducibility .
	manualset3
134463	4	406374	13	NULL	NULL	0	NULL	methods	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of relative standard deviations did not exceed 1.6 % , indicating that the proposed methods having good repeatability and reproducibility .
	manualset3
134464	5	406374	13	NULL	NULL	0	NULL	repeatability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of relative standard deviations did not exceed 1.6 % , indicating that the proposed methods having good repeatability and reproducibility .
	manualset3
134465	6	406374	13	NULL	NULL	0	NULL	reproducibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of relative standard deviations did not exceed 1.6 % , indicating that the proposed methods having good repeatability and reproducibility .
	manualset3
134466	1	406375	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of spin relaxation time measurements have been analyzed using the model-free formalism and completed by dispersion relaxation measurements .
	manualset3
134467	2	406375	13	NULL	NULL	0	NULL	spin relaxation time measurements 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of spin relaxation time measurements have been analyzed using the model-free formalism and completed by dispersion relaxation measurements .
	manualset3
134468	3	406375	13	NULL	NULL	0	NULL	model-free formalism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of spin relaxation time measurements have been analyzed using the model-free formalism and completed by dispersion relaxation measurements .
	manualset3
134469	4	406375	13	NULL	NULL	0	NULL	dispersion relaxation measurements	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of spin relaxation time measurements have been analyzed using the model-free formalism and completed by dispersion relaxation measurements .
	manualset3
134470	1	406376	13	NULL	NULL	0	NULL	Results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of tail-flick and formalin tests demonstrated a dose-dependent analgesic effects for WIN55 , 212-2 , with the most significant response at the dose of 20g/side .
	manualset3
134471	2	406376	13	NULL	NULL	0	NULL	tail-flick test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of tail-flick and formalin tests demonstrated a dose-dependent analgesic effects for WIN55 , 212-2 , with the most significant response at the dose of 20g/side .
	manualset3
134472	3	406376	13	NULL	NULL	0	NULL	formalin test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of tail-flick and formalin tests demonstrated a dose-dependent analgesic effects for WIN55 , 212-2 , with the most significant response at the dose of 20g/side .
	manualset3
134473	4	406376	13	NULL	NULL	0	NULL	dose-dependent analgesic effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of tail-flick and formalin tests demonstrated a dose-dependent analgesic effects for WIN55 , 212-2 , with the most significant response at the dose of 20g/side .
	manualset3
134474	5	406376	13	NULL	NULL	0	NULL	WIN55 , 212-2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of tail-flick and formalin tests demonstrated a dose-dependent analgesic effects for WIN55 , 212-2 , with the most significant response at the dose of 20g/side .
	manualset3
134475	6	406376	13	NULL	NULL	0	NULL	response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of tail-flick and formalin tests demonstrated a dose-dependent analgesic effects for WIN55 , 212-2 , with the most significant response at the dose of 20g/side .
	manualset3
134476	7	406376	13	NULL	NULL	0	NULL	dose of 20g/side	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of tail-flick and formalin tests demonstrated a dose-dependent analgesic effects for WIN55 , 212-2 , with the most significant response at the dose of 20g/side .
	manualset3
134477	1	406377	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of the batch experiments showed an effective removal ( 99.5 % ) of arsenic compounds from the synthetic water samples .
	manualset3
134478	2	406377	13	NULL	NULL	0	NULL	batch experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of the batch experiments showed an effective removal ( 99.5 % ) of arsenic compounds from the synthetic water samples .
	manualset3
134479	3	406377	13	NULL	NULL	0	NULL	effective removal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of the batch experiments showed an effective removal ( 99.5 % ) of arsenic compounds from the synthetic water samples .
	manualset3
134480	4	406377	13	NULL	NULL	0	NULL	99.5 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of the batch experiments showed an effective removal ( 99.5 % ) of arsenic compounds from the synthetic water samples .
	manualset3
134481	5	406377	13	NULL	NULL	0	NULL	arsenic compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of the batch experiments showed an effective removal ( 99.5 % ) of arsenic compounds from the synthetic water samples .
	manualset3
134482	6	406377	13	NULL	NULL	0	NULL	synthetic water samples 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of the batch experiments showed an effective removal ( 99.5 % ) of arsenic compounds from the synthetic water samples .
	manualset3
134483	1	406378	13	NULL	NULL	0	NULL	Results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of the first 90 patients to have sleep nasendoscopy are presented .
	manualset3
134484	2	406378	13	NULL	NULL	0	NULL	first 90 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of the first 90 patients to have sleep nasendoscopy are presented .
	manualset3
134485	3	406378	13	NULL	NULL	NULL	NULL	sleep nasendoscopy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Results of the first 90 patients to have sleep nasendoscopy are presented .
	manualset3
134486	1	406379	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of two-choice huddling tests indicated that daily , 4-hr exposures to a perfumed foster dam induced filial preferences for odors associated with maternal care .
	manualset3
134487	2	406379	13	NULL	NULL	0	NULL	two-choice huddling tests	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of two-choice huddling tests indicated that daily , 4-hr exposures to a perfumed foster dam induced filial preferences for odors associated with maternal care .
	manualset3
134488	3	406379	13	NULL	NULL	NULL	NULL	4-hr	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Results of two-choice huddling tests indicated that daily , 4-hr exposures to a perfumed foster dam induced filial preferences for odors associated with maternal care .
	manualset3
134489	4	406379	13	NULL	NULL	0	NULL	perfumed foster dam	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of two-choice huddling tests indicated that daily , 4-hr exposures to a perfumed foster dam induced filial preferences for odors associated with maternal care .
	manualset3
134490	5	406379	13	NULL	NULL	NULL	NULL	filial preferences	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Results of two-choice huddling tests indicated that daily , 4-hr exposures to a perfumed foster dam induced filial preferences for odors associated with maternal care .
	manualset3
134491	6	406379	13	NULL	NULL	0	NULL	odors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of two-choice huddling tests indicated that daily , 4-hr exposures to a perfumed foster dam induced filial preferences for odors associated with maternal care .
	manualset3
134492	7	406379	13	NULL	NULL	0	NULL	maternal care	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of two-choice huddling tests indicated that daily , 4-hr exposures to a perfumed foster dam induced filial preferences for odors associated with maternal care .
	manualset3
134493	8	406379	13	NULL	NULL	0	NULL	exposures 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of two-choice huddling tests indicated that daily , 4-hr exposures to a perfumed foster dam induced filial preferences for odors associated with maternal care .
	manualset3
134494	1	406380	13	NULL	NULL	0	NULL	negative correlation coefficient	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A negative correlation coefficient ( -0.3 ) between PPAR relative gene expression and liver tissue fat content confirm the anti-lipogenic effect of PPAR , however , the change in these parameters was not completely parallel .
	manualset3
134495	2	406380	13	NULL	NULL	0	NULL	-0.3	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A negative correlation coefficient ( -0.3 ) between PPAR relative gene expression and liver tissue fat content confirm the anti-lipogenic effect of PPAR , however , the change in these parameters was not completely parallel .
	manualset3
134496	3	406380	13	NULL	NULL	0	NULL	PPAR relative gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A negative correlation coefficient ( -0.3 ) between PPAR relative gene expression and liver tissue fat content confirm the anti-lipogenic effect of PPAR , however , the change in these parameters was not completely parallel .
	manualset3
134497	4	406380	13	NULL	NULL	0	NULL	liver tissue fat content 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A negative correlation coefficient ( -0.3 ) between PPAR relative gene expression and liver tissue fat content confirm the anti-lipogenic effect of PPAR , however , the change in these parameters was not completely parallel .
	manualset3
134498	5	406380	13	NULL	NULL	0	NULL	anti-lipogenic effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A negative correlation coefficient ( -0.3 ) between PPAR relative gene expression and liver tissue fat content confirm the anti-lipogenic effect of PPAR , however , the change in these parameters was not completely parallel .
	manualset3
134499	6	406380	13	NULL	NULL	0	NULL	PPAR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A negative correlation coefficient ( -0.3 ) between PPAR relative gene expression and liver tissue fat content confirm the anti-lipogenic effect of PPAR , however , the change in these parameters was not completely parallel .
	manualset3
134500	7	406380	13	NULL	NULL	0	NULL	change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A negative correlation coefficient ( -0.3 ) between PPAR relative gene expression and liver tissue fat content confirm the anti-lipogenic effect of PPAR , however , the change in these parameters was not completely parallel .
	manualset3
134501	8	406380	13	NULL	NULL	0	NULL	parameters	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A negative correlation coefficient ( -0.3 ) between PPAR relative gene expression and liver tissue fat content confirm the anti-lipogenic effect of PPAR , however , the change in these parameters was not completely parallel .
	manualset3
134502	1	406381	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results on the effects of various decision parameters used in hotspot identification procedures are discussed .
	manualset3
134503	2	406381	13	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results on the effects of various decision parameters used in hotspot identification procedures are discussed .
	manualset3
134504	3	406381	13	NULL	NULL	0	NULL	various decision parameters	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results on the effects of various decision parameters used in hotspot identification procedures are discussed .
	manualset3
134505	4	406381	13	NULL	NULL	0	NULL	hotspot identification procedures 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results on the effects of various decision parameters used in hotspot identification procedures are discussed .
	manualset3
134506	1	406382	13	NULL	NULL	NULL	NULL	Results 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Results point to the importance of understanding the meaning that religion has to the families in the health-disease process , so nurses can work on the promotion of health .
	manualset3
134507	2	406382	13	NULL	NULL	0	NULL	importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results point to the importance of understanding the meaning that religion has to the families in the health-disease process , so nurses can work on the promotion of health .
	manualset3
134508	3	406382	13	NULL	NULL	0	NULL	religion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results point to the importance of understanding the meaning that religion has to the families in the health-disease process , so nurses can work on the promotion of health .
	manualset3
134509	4	406382	13	NULL	NULL	0	NULL	families 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results point to the importance of understanding the meaning that religion has to the families in the health-disease process , so nurses can work on the promotion of health .
	manualset3
134510	5	406382	13	NULL	NULL	0	NULL	health-disease process	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results point to the importance of understanding the meaning that religion has to the families in the health-disease process , so nurses can work on the promotion of health .
	manualset3
134511	6	406382	13	NULL	NULL	0	NULL	nurses	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results point to the importance of understanding the meaning that religion has to the families in the health-disease process , so nurses can work on the promotion of health .
	manualset3
134512	7	406382	13	NULL	NULL	0	NULL	promotion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results point to the importance of understanding the meaning that religion has to the families in the health-disease process , so nurses can work on the promotion of health .
	manualset3
134513	8	406382	13	NULL	NULL	0	NULL	health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results point to the importance of understanding the meaning that religion has to the families in the health-disease process , so nurses can work on the promotion of health .
	manualset3
138434	9	406382	13	NULL	NULL	0	NULL	meaning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results point to the importance of understanding the meaning that religion has to the families in the health-disease process , so nurses can work on the promotion of health .
	manualset3
134514	1	406383	13	NULL	NULL	0	NULL	Results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results revealed that , 20 months after implementation , the ban was respected by about one out of seven retailers and compliance did not improve significantly over the following 24-month period .
	manualset3
134515	2	406383	13	NULL	NULL	0	NULL	20 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Results revealed that , 20 months after implementation , the ban was respected by about one out of seven retailers and compliance did not improve significantly over the following 24-month period .
	manualset3
134516	3	406383	13	NULL	NULL	0	NULL	implementation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results revealed that , 20 months after implementation , the ban was respected by about one out of seven retailers and compliance did not improve significantly over the following 24-month period .
	manualset3
134517	4	406383	13	NULL	NULL	0	NULL	ban	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results revealed that , 20 months after implementation , the ban was respected by about one out of seven retailers and compliance did not improve significantly over the following 24-month period .
	manualset3
134518	5	406383	13	NULL	NULL	0	NULL	one out of seven retailers	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results revealed that , 20 months after implementation , the ban was respected by about one out of seven retailers and compliance did not improve significantly over the following 24-month period .
	manualset3
134519	6	406383	13	NULL	NULL	0	NULL	compliance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results revealed that , 20 months after implementation , the ban was respected by about one out of seven retailers and compliance did not improve significantly over the following 24-month period .
	manualset3
134520	7	406383	13	NULL	NULL	0	NULL	24-month period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Results revealed that , 20 months after implementation , the ban was respected by about one out of seven retailers and compliance did not improve significantly over the following 24-month period .
	manualset3
134521	1	406384	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results show that , in the resting conditions , J ( glucose ) from all exogenous substrates was significantly higher ( P & lt ; 0.01 ) in PP-H than in PV-H .
	manualset3
134522	2	406384	13	NULL	NULL	0	NULL	resting conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Results show that , in the resting conditions , J ( glucose ) from all exogenous substrates was significantly higher ( P & lt ; 0.01 ) in PP-H than in PV-H .
	manualset3
134523	3	406384	13	NULL	NULL	0	NULL	J ( glucose )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results show that , in the resting conditions , J ( glucose ) from all exogenous substrates was significantly higher ( P & lt ; 0.01 ) in PP-H than in PV-H .
	manualset3
134524	4	406384	13	NULL	NULL	0	NULL	exogenous substrates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results show that , in the resting conditions , J ( glucose ) from all exogenous substrates was significantly higher ( P & lt ; 0.01 ) in PP-H than in PV-H .
	manualset3
134525	5	406384	13	NULL	NULL	0	NULL	P & lt ; 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results show that , in the resting conditions , J ( glucose ) from all exogenous substrates was significantly higher ( P & lt ; 0.01 ) in PP-H than in PV-H .
	manualset3
134526	6	406384	13	NULL	NULL	0	NULL	PP-H	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Results show that , in the resting conditions , J ( glucose ) from all exogenous substrates was significantly higher ( P & lt ; 0.01 ) in PP-H than in PV-H .
	manualset3
134527	7	406384	13	NULL	NULL	0	NULL	PV-H	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Results show that , in the resting conditions , J ( glucose ) from all exogenous substrates was significantly higher ( P & lt ; 0.01 ) in PP-H than in PV-H .
	manualset3
134528	1	406385	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results show that agonist muscle activity and antagonist muscle co-activity levels are significantly greater in isotonic mode compared to isokinetic mode .
	manualset3
134529	2	406385	13	NULL	NULL	NULL	NULL	agonist muscle activity levels	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Results show that agonist muscle activity and antagonist muscle co-activity levels are significantly greater in isotonic mode compared to isokinetic mode .
	manualset3
134530	3	406385	13	NULL	NULL	0	NULL	antagonist muscle co-activity levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results show that agonist muscle activity and antagonist muscle co-activity levels are significantly greater in isotonic mode compared to isokinetic mode .
	manualset3
134531	4	406385	13	NULL	NULL	0	NULL	isotonic mode	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results show that agonist muscle activity and antagonist muscle co-activity levels are significantly greater in isotonic mode compared to isokinetic mode .
	manualset3
134532	5	406385	13	NULL	NULL	0	NULL	isokinetic mode 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results show that agonist muscle activity and antagonist muscle co-activity levels are significantly greater in isotonic mode compared to isokinetic mode .
	manualset3
134533	1	406386	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results show that only bacterial soluble factors that increase cell-surface galactose namely , those of Bacteroides thetaiotaomicron and Lactobacillus casei were able to efficiently block rotavirus infections .
	manualset3
134534	2	406386	13	NULL	NULL	0	NULL	bacterial soluble factors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results show that only bacterial soluble factors that increase cell-surface galactose namely , those of Bacteroides thetaiotaomicron and Lactobacillus casei were able to efficiently block rotavirus infections .
	manualset3
134535	3	406386	13	NULL	NULL	0	NULL	cell-surface galactose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results show that only bacterial soluble factors that increase cell-surface galactose namely , those of Bacteroides thetaiotaomicron and Lactobacillus casei were able to efficiently block rotavirus infections .
	manualset3
134536	4	406386	13	NULL	NULL	0	NULL	Bacteroides thetaiotaomicron	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Results show that only bacterial soluble factors that increase cell-surface galactose namely , those of Bacteroides thetaiotaomicron and Lactobacillus casei were able to efficiently block rotavirus infections .
	manualset3
134537	5	406386	13	NULL	NULL	0	NULL	Lactobacillus casei	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Results show that only bacterial soluble factors that increase cell-surface galactose namely , those of Bacteroides thetaiotaomicron and Lactobacillus casei were able to efficiently block rotavirus infections .
	manualset3
134538	6	406386	13	NULL	NULL	0	NULL	rotavirus infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results show that only bacterial soluble factors that increase cell-surface galactose namely , those of Bacteroides thetaiotaomicron and Lactobacillus casei were able to efficiently block rotavirus infections .
	manualset3
134539	1	406387	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that , in contrast to blood samples from HDs , freshly isolated PBMCs from un treated HCL patients did not express IFN-alpha mRNA , whereas IFN-alpha transcripts were found in patients who were under rhIFN-alpha therapy Plasma of untreated patients contained no , or extremely low levels of IFN-alpha as compared with plasma of treated patients and HDs .
	manualset3
134540	2	406387	13	NULL	NULL	0	NULL	contrast	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that , in contrast to blood samples from HDs , freshly isolated PBMCs from un treated HCL patients did not express IFN-alpha mRNA , whereas IFN-alpha transcripts were found in patients who were under rhIFN-alpha therapy Plasma of untreated patients contained no , or extremely low levels of IFN-alpha as compared with plasma of treated patients and HDs .
	manualset3
134541	3	406387	13	NULL	NULL	0	NULL	blood samples	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that , in contrast to blood samples from HDs , freshly isolated PBMCs from un treated HCL patients did not express IFN-alpha mRNA , whereas IFN-alpha transcripts were found in patients who were under rhIFN-alpha therapy Plasma of untreated patients contained no , or extremely low levels of IFN-alpha as compared with plasma of treated patients and HDs .
	manualset3
134542	4	406387	13	NULL	NULL	0	NULL	HDs	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that , in contrast to blood samples from HDs , freshly isolated PBMCs from un treated HCL patients did not express IFN-alpha mRNA , whereas IFN-alpha transcripts were found in patients who were under rhIFN-alpha therapy Plasma of untreated patients contained no , or extremely low levels of IFN-alpha as compared with plasma of treated patients and HDs .
	manualset3
134543	5	406387	13	NULL	NULL	0	NULL	PBMCs 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that , in contrast to blood samples from HDs , freshly isolated PBMCs from un treated HCL patients did not express IFN-alpha mRNA , whereas IFN-alpha transcripts were found in patients who were under rhIFN-alpha therapy Plasma of untreated patients contained no , or extremely low levels of IFN-alpha as compared with plasma of treated patients and HDs .
	manualset3
134544	6	406387	13	NULL	NULL	0	NULL	HCL patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that , in contrast to blood samples from HDs , freshly isolated PBMCs from un treated HCL patients did not express IFN-alpha mRNA , whereas IFN-alpha transcripts were found in patients who were under rhIFN-alpha therapy Plasma of untreated patients contained no , or extremely low levels of IFN-alpha as compared with plasma of treated patients and HDs .
	manualset3
134545	7	406387	13	NULL	NULL	0	NULL	IFN-alpha mRNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that , in contrast to blood samples from HDs , freshly isolated PBMCs from un treated HCL patients did not express IFN-alpha mRNA , whereas IFN-alpha transcripts were found in patients who were under rhIFN-alpha therapy Plasma of untreated patients contained no , or extremely low levels of IFN-alpha as compared with plasma of treated patients and HDs .
	manualset3
134546	8	406387	13	NULL	NULL	0	NULL	IFN-alpha transcripts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that , in contrast to blood samples from HDs , freshly isolated PBMCs from un treated HCL patients did not express IFN-alpha mRNA , whereas IFN-alpha transcripts were found in patients who were under rhIFN-alpha therapy Plasma of untreated patients contained no , or extremely low levels of IFN-alpha as compared with plasma of treated patients and HDs .
	manualset3
134547	9	406387	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that , in contrast to blood samples from HDs , freshly isolated PBMCs from un treated HCL patients did not express IFN-alpha mRNA , whereas IFN-alpha transcripts were found in patients who were under rhIFN-alpha therapy Plasma of untreated patients contained no , or extremely low levels of IFN-alpha as compared with plasma of treated patients and HDs .
	manualset3
134548	10	406387	13	NULL	NULL	0	NULL	rhIFN-alpha therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that , in contrast to blood samples from HDs , freshly isolated PBMCs from un treated HCL patients did not express IFN-alpha mRNA , whereas IFN-alpha transcripts were found in patients who were under rhIFN-alpha therapy Plasma of untreated patients contained no , or extremely low levels of IFN-alpha as compared with plasma of treated patients and HDs .
	manualset3
134549	11	406387	13	NULL	NULL	NULL	NULL	Plasma	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Results showed that , in contrast to blood samples from HDs , freshly isolated PBMCs from un treated HCL patients did not express IFN-alpha mRNA , whereas IFN-alpha transcripts were found in patients who were under rhIFN-alpha therapy Plasma of untreated patients contained no , or extremely low levels of IFN-alpha as compared with plasma of treated patients and HDs .
	manualset3
134550	12	406387	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that , in contrast to blood samples from HDs , freshly isolated PBMCs from un treated HCL patients did not express IFN-alpha mRNA , whereas IFN-alpha transcripts were found in patients who were under rhIFN-alpha therapy Plasma of untreated patients contained no , or extremely low levels of IFN-alpha as compared with plasma of treated patients and HDs .
	manualset3
134551	13	406387	13	NULL	NULL	0	NULL	levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that , in contrast to blood samples from HDs , freshly isolated PBMCs from un treated HCL patients did not express IFN-alpha mRNA , whereas IFN-alpha transcripts were found in patients who were under rhIFN-alpha therapy Plasma of untreated patients contained no , or extremely low levels of IFN-alpha as compared with plasma of treated patients and HDs .
	manualset3
134552	14	406387	13	NULL	NULL	0	NULL	IFN-alpha 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that , in contrast to blood samples from HDs , freshly isolated PBMCs from un treated HCL patients did not express IFN-alpha mRNA , whereas IFN-alpha transcripts were found in patients who were under rhIFN-alpha therapy Plasma of untreated patients contained no , or extremely low levels of IFN-alpha as compared with plasma of treated patients and HDs .
	manualset3
134553	15	406387	13	NULL	NULL	NULL	NULL	plasma	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Results showed that , in contrast to blood samples from HDs , freshly isolated PBMCs from un treated HCL patients did not express IFN-alpha mRNA , whereas IFN-alpha transcripts were found in patients who were under rhIFN-alpha therapy Plasma of untreated patients contained no , or extremely low levels of IFN-alpha as compared with plasma of treated patients and HDs .
	manualset3
134554	16	406387	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that , in contrast to blood samples from HDs , freshly isolated PBMCs from un treated HCL patients did not express IFN-alpha mRNA , whereas IFN-alpha transcripts were found in patients who were under rhIFN-alpha therapy Plasma of untreated patients contained no , or extremely low levels of IFN-alpha as compared with plasma of treated patients and HDs .
	manualset3
134555	17	406387	13	NULL	NULL	0	NULL	HDs	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that , in contrast to blood samples from HDs , freshly isolated PBMCs from un treated HCL patients did not express IFN-alpha mRNA , whereas IFN-alpha transcripts were found in patients who were under rhIFN-alpha therapy Plasma of untreated patients contained no , or extremely low levels of IFN-alpha as compared with plasma of treated patients and HDs .
	manualset3
134556	1	406388	13	NULL	NULL	0	NULL	Results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that 211 ( 79.6 % ) knew fecal-oral route as the commonest mode for poliovirus transmission , 231 ( 87.2 % ) knew the age for vaccination , 224 ( 84.5 % ) knew the correct use of vaccine vial monitor while 143 ( 53.9 % ) knew the correct action to take when a case of polio was identified .
	manualset3
134557	2	406388	13	NULL	NULL	0	NULL	211 ( 79.6 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that 211 ( 79.6 % ) knew fecal-oral route as the commonest mode for poliovirus transmission , 231 ( 87.2 % ) knew the age for vaccination , 224 ( 84.5 % ) knew the correct use of vaccine vial monitor while 143 ( 53.9 % ) knew the correct action to take when a case of polio was identified .
	manualset3
134558	3	406388	13	NULL	NULL	0	NULL	fecal-oral route	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that 211 ( 79.6 % ) knew fecal-oral route as the commonest mode for poliovirus transmission , 231 ( 87.2 % ) knew the age for vaccination , 224 ( 84.5 % ) knew the correct use of vaccine vial monitor while 143 ( 53.9 % ) knew the correct action to take when a case of polio was identified .
	manualset3
134559	4	406388	13	NULL	NULL	0	NULL	commonest mode	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that 211 ( 79.6 % ) knew fecal-oral route as the commonest mode for poliovirus transmission , 231 ( 87.2 % ) knew the age for vaccination , 224 ( 84.5 % ) knew the correct use of vaccine vial monitor while 143 ( 53.9 % ) knew the correct action to take when a case of polio was identified .
	manualset3
134560	5	406388	13	NULL	NULL	0	NULL	poliovirus transmission	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that 211 ( 79.6 % ) knew fecal-oral route as the commonest mode for poliovirus transmission , 231 ( 87.2 % ) knew the age for vaccination , 224 ( 84.5 % ) knew the correct use of vaccine vial monitor while 143 ( 53.9 % ) knew the correct action to take when a case of polio was identified .
	manualset3
134561	6	406388	13	NULL	NULL	0	NULL	231 ( 87.2 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that 211 ( 79.6 % ) knew fecal-oral route as the commonest mode for poliovirus transmission , 231 ( 87.2 % ) knew the age for vaccination , 224 ( 84.5 % ) knew the correct use of vaccine vial monitor while 143 ( 53.9 % ) knew the correct action to take when a case of polio was identified .
	manualset3
134562	7	406388	13	NULL	NULL	0	NULL	age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that 211 ( 79.6 % ) knew fecal-oral route as the commonest mode for poliovirus transmission , 231 ( 87.2 % ) knew the age for vaccination , 224 ( 84.5 % ) knew the correct use of vaccine vial monitor while 143 ( 53.9 % ) knew the correct action to take when a case of polio was identified .
	manualset3
134563	8	406388	13	NULL	NULL	0	NULL	vaccination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that 211 ( 79.6 % ) knew fecal-oral route as the commonest mode for poliovirus transmission , 231 ( 87.2 % ) knew the age for vaccination , 224 ( 84.5 % ) knew the correct use of vaccine vial monitor while 143 ( 53.9 % ) knew the correct action to take when a case of polio was identified .
	manualset3
134564	9	406388	13	NULL	NULL	0	NULL	224 ( 84.5 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that 211 ( 79.6 % ) knew fecal-oral route as the commonest mode for poliovirus transmission , 231 ( 87.2 % ) knew the age for vaccination , 224 ( 84.5 % ) knew the correct use of vaccine vial monitor while 143 ( 53.9 % ) knew the correct action to take when a case of polio was identified .
	manualset3
134565	9	406388	13	NULL	NULL	NULL	NULL	vaccine vial monitor	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Results showed that 211 ( 79.6 % ) knew fecal-oral route as the commonest mode for poliovirus transmission , 231 ( 87.2 % ) knew the age for vaccination , 224 ( 84.5 % ) knew the correct use of vaccine vial monitor while 143 ( 53.9 % ) knew the correct action to take when a case of polio was identified .
	manualset3
134566	10	406388	13	NULL	NULL	0	NULL	143 ( 53.9 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that 211 ( 79.6 % ) knew fecal-oral route as the commonest mode for poliovirus transmission , 231 ( 87.2 % ) knew the age for vaccination , 224 ( 84.5 % ) knew the correct use of vaccine vial monitor while 143 ( 53.9 % ) knew the correct action to take when a case of polio was identified .
	manualset3
134567	11	406388	13	NULL	NULL	0	NULL	action	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that 211 ( 79.6 % ) knew fecal-oral route as the commonest mode for poliovirus transmission , 231 ( 87.2 % ) knew the age for vaccination , 224 ( 84.5 % ) knew the correct use of vaccine vial monitor while 143 ( 53.9 % ) knew the correct action to take when a case of polio was identified .
	manualset3
134568	12	406388	13	NULL	NULL	0	NULL	case of polio	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that 211 ( 79.6 % ) knew fecal-oral route as the commonest mode for poliovirus transmission , 231 ( 87.2 % ) knew the age for vaccination , 224 ( 84.5 % ) knew the correct use of vaccine vial monitor while 143 ( 53.9 % ) knew the correct action to take when a case of polio was identified .
	manualset3
134569	1	406389	13	NULL	NULL	0	NULL	Results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that differentiated oligodendrocytes , which express both MBP and GC , are able to proliferate .
	manualset3
134570	2	406389	13	NULL	NULL	0	NULL	differentiated oligodendrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that differentiated oligodendrocytes , which express both MBP and GC , are able to proliferate .
	manualset3
134571	3	406389	13	NULL	NULL	0	NULL	MBP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that differentiated oligodendrocytes , which express both MBP and GC , are able to proliferate .
	manualset3
134572	4	406389	13	NULL	NULL	0	NULL	GC	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that differentiated oligodendrocytes , which express both MBP and GC , are able to proliferate .
	manualset3
134573	1	406390	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that food intake was significantly less in the cholesterol-fed group , while requirements for maintenance and for liveweight gain , as adjusted to metabolic body size ( Wkg-0 .75 ) , were not significantly different .
	manualset3
134574	2	406390	13	NULL	NULL	0	NULL	food intake 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that food intake was significantly less in the cholesterol-fed group , while requirements for maintenance and for liveweight gain , as adjusted to metabolic body size ( Wkg-0 .75 ) , were not significantly different .
	manualset3
134575	3	406390	13	NULL	NULL	0	NULL	cholesterol-fed group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that food intake was significantly less in the cholesterol-fed group , while requirements for maintenance and for liveweight gain , as adjusted to metabolic body size ( Wkg-0 .75 ) , were not significantly different .
	manualset3
134576	4	406390	13	NULL	NULL	0	NULL	requirements 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that food intake was significantly less in the cholesterol-fed group , while requirements for maintenance and for liveweight gain , as adjusted to metabolic body size ( Wkg-0 .75 ) , were not significantly different .
	manualset3
134577	5	406390	13	NULL	NULL	0	NULL	maintenance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that food intake was significantly less in the cholesterol-fed group , while requirements for maintenance and for liveweight gain , as adjusted to metabolic body size ( Wkg-0 .75 ) , were not significantly different .
	manualset3
134578	6	406390	13	NULL	NULL	0	NULL	liveweight gain	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that food intake was significantly less in the cholesterol-fed group , while requirements for maintenance and for liveweight gain , as adjusted to metabolic body size ( Wkg-0 .75 ) , were not significantly different .
	manualset3
134579	7	406390	13	NULL	NULL	0	NULL	metabolic body size	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that food intake was significantly less in the cholesterol-fed group , while requirements for maintenance and for liveweight gain , as adjusted to metabolic body size ( Wkg-0 .75 ) , were not significantly different .
	manualset3
134580	8	406390	13	NULL	NULL	0	NULL	Wkg-0 .75	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that food intake was significantly less in the cholesterol-fed group , while requirements for maintenance and for liveweight gain , as adjusted to metabolic body size ( Wkg-0 .75 ) , were not significantly different .
	manualset3
134581	1	406391	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that nitric oxide alone had no effect on gelatinase A activity relative to control , whereas superoxide-derived metabolites increased activity .
	manualset3
134582	2	406391	13	NULL	NULL	0	NULL	nitric oxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that nitric oxide alone had no effect on gelatinase A activity relative to control , whereas superoxide-derived metabolites increased activity .
	manualset3
134583	3	406391	13	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that nitric oxide alone had no effect on gelatinase A activity relative to control , whereas superoxide-derived metabolites increased activity .
	manualset3
134584	4	406391	13	NULL	NULL	0	NULL	gelatinase A activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that nitric oxide alone had no effect on gelatinase A activity relative to control , whereas superoxide-derived metabolites increased activity .
	manualset3
134585	5	406391	13	NULL	NULL	0	NULL	control	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that nitric oxide alone had no effect on gelatinase A activity relative to control , whereas superoxide-derived metabolites increased activity .
	manualset3
134586	6	406391	13	NULL	NULL	0	NULL	superoxide-derived metabolites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that nitric oxide alone had no effect on gelatinase A activity relative to control , whereas superoxide-derived metabolites increased activity .
	manualset3
134587	7	406391	13	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that nitric oxide alone had no effect on gelatinase A activity relative to control , whereas superoxide-derived metabolites increased activity .
	manualset3
134588	1	406392	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that speech recognition scores dropped because of noise and spectral shifting , and that the interactive effects of spectral shifting and background conditions depended on the degree/type of spectral shift , background conditions , and the speech test materials .
	manualset3
134589	2	406392	13	NULL	NULL	0	NULL	speech recognition scores	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that speech recognition scores dropped because of noise and spectral shifting , and that the interactive effects of spectral shifting and background conditions depended on the degree/type of spectral shift , background conditions , and the speech test materials .
	manualset3
134590	3	406392	13	NULL	NULL	0	NULL	noise 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that speech recognition scores dropped because of noise and spectral shifting , and that the interactive effects of spectral shifting and background conditions depended on the degree/type of spectral shift , background conditions , and the speech test materials .
	manualset3
134591	4	406392	13	NULL	NULL	0	NULL	interactive effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that speech recognition scores dropped because of noise and spectral shifting , and that the interactive effects of spectral shifting and background conditions depended on the degree/type of spectral shift , background conditions , and the speech test materials .
	manualset3
134592	5	406392	13	NULL	NULL	0	NULL	background conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that speech recognition scores dropped because of noise and spectral shifting , and that the interactive effects of spectral shifting and background conditions depended on the degree/type of spectral shift , background conditions , and the speech test materials .
	manualset3
134593	6	406392	13	NULL	NULL	0	NULL	degree/type of spectral shift	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that speech recognition scores dropped because of noise and spectral shifting , and that the interactive effects of spectral shifting and background conditions depended on the degree/type of spectral shift , background conditions , and the speech test materials .
	manualset3
134594	7	406392	13	NULL	NULL	0	NULL	background conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that speech recognition scores dropped because of noise and spectral shifting , and that the interactive effects of spectral shifting and background conditions depended on the degree/type of spectral shift , background conditions , and the speech test materials .
	manualset3
134595	8	406392	13	NULL	NULL	0	NULL	speech test materials	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that speech recognition scores dropped because of noise and spectral shifting , and that the interactive effects of spectral shifting and background conditions depended on the degree/type of spectral shift , background conditions , and the speech test materials .
	manualset3
138435	9	406392	13	NULL	NULL	0	NULL	spectral shifting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that speech recognition scores dropped because of noise and spectral shifting , and that the interactive effects of spectral shifting and background conditions depended on the degree/type of spectral shift , background conditions , and the speech test materials .
	manualset3
134596	1	406393	13	NULL	NULL	NULL	NULL	Results 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Results showed that the presence of heavy metals and cationic surfactants caused a significant increase on the BPA sorption .
	manualset3
134597	2	406393	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that the presence of heavy metals and cationic surfactants caused a significant increase on the BPA sorption .
	manualset3
134598	3	406393	13	NULL	NULL	0	NULL	heavy metals 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that the presence of heavy metals and cationic surfactants caused a significant increase on the BPA sorption .
	manualset3
134599	4	406393	13	NULL	NULL	NULL	NULL	cationic surfactants	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Results showed that the presence of heavy metals and cationic surfactants caused a significant increase on the BPA sorption .
	manualset3
134600	5	406393	13	NULL	NULL	0	NULL	BPA sorption 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that the presence of heavy metals and cationic surfactants caused a significant increase on the BPA sorption .
	manualset3
134601	1	406394	13	NULL	NULL	0	NULL	Results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that the yield is strongly dependent on the nature of the interlayer anion in the hydrotalcite structure .
	manualset3
134602	2	406394	13	NULL	NULL	0	NULL	yield	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that the yield is strongly dependent on the nature of the interlayer anion in the hydrotalcite structure .
	manualset3
134603	3	406394	13	NULL	NULL	0	NULL	nature	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that the yield is strongly dependent on the nature of the interlayer anion in the hydrotalcite structure .
	manualset3
134604	4	406394	13	NULL	NULL	0	NULL	interlayer anion	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that the yield is strongly dependent on the nature of the interlayer anion in the hydrotalcite structure .
	manualset3
134605	5	406394	13	NULL	NULL	0	NULL	hydrotalcite structure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results showed that the yield is strongly dependent on the nature of the interlayer anion in the hydrotalcite structure .
	manualset3
134606	1	406395	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that , up to now , there is no definite proof of qualitatively different mechanisms underlying the processing of upright and inverted faces , respectively .
	manualset3
134607	2	406395	13	NULL	NULL	0	NULL	proof	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that , up to now , there is no definite proof of qualitatively different mechanisms underlying the processing of upright and inverted faces , respectively .
	manualset3
134608	3	406395	13	NULL	NULL	0	NULL	mechanisms 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that , up to now , there is no definite proof of qualitatively different mechanisms underlying the processing of upright and inverted faces , respectively .
	manualset3
134609	4	406395	13	NULL	NULL	NULL	NULL	upright faces	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Results suggest that , up to now , there is no definite proof of qualitatively different mechanisms underlying the processing of upright and inverted faces , respectively .
	manualset3
134610	5	406395	13	NULL	NULL	0	NULL	inverted faces 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that , up to now , there is no definite proof of qualitatively different mechanisms underlying the processing of upright and inverted faces , respectively .
	manualset3
134611	1	406396	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that deep as well as mild hypothermia decreased hypoxia-induced hyperpermeability by lowering the expression of the permeability-increasing protein VEGF and with it the release of NO .
	manualset3
134612	2	406396	13	NULL	NULL	0	NULL	mild hypothermia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that deep as well as mild hypothermia decreased hypoxia-induced hyperpermeability by lowering the expression of the permeability-increasing protein VEGF and with it the release of NO .
	manualset3
134613	3	406396	13	NULL	NULL	0	NULL	hyperpermeability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that deep as well as mild hypothermia decreased hypoxia-induced hyperpermeability by lowering the expression of the permeability-increasing protein VEGF and with it the release of NO .
	manualset3
134614	4	406396	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that deep as well as mild hypothermia decreased hypoxia-induced hyperpermeability by lowering the expression of the permeability-increasing protein VEGF and with it the release of NO .
	manualset3
134615	5	406396	13	NULL	NULL	0	NULL	permeability-increasing protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that deep as well as mild hypothermia decreased hypoxia-induced hyperpermeability by lowering the expression of the permeability-increasing protein VEGF and with it the release of NO .
	manualset3
134616	6	406396	13	NULL	NULL	0	NULL	VEGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that deep as well as mild hypothermia decreased hypoxia-induced hyperpermeability by lowering the expression of the permeability-increasing protein VEGF and with it the release of NO .
	manualset3
134617	7	406396	13	NULL	NULL	0	NULL	release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that deep as well as mild hypothermia decreased hypoxia-induced hyperpermeability by lowering the expression of the permeability-increasing protein VEGF and with it the release of NO .
	manualset3
134618	8	406396	13	NULL	NULL	0	NULL	NO 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that deep as well as mild hypothermia decreased hypoxia-induced hyperpermeability by lowering the expression of the permeability-increasing protein VEGF and with it the release of NO .
	manualset3
134619	1	406397	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that the CD-ROM is no substitute for real life , hands on experience , although when used as an adjunct to traditional teaching methods , it can enhance learning .
	manualset3
134620	2	406397	13	NULL	NULL	0	NULL	CD-ROM	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that the CD-ROM is no substitute for real life , hands on experience , although when used as an adjunct to traditional teaching methods , it can enhance learning .
	manualset3
134621	3	406397	13	NULL	NULL	0	NULL	substitute	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that the CD-ROM is no substitute for real life , hands on experience , although when used as an adjunct to traditional teaching methods , it can enhance learning .
	manualset3
134622	4	406397	13	NULL	NULL	0	NULL	real life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that the CD-ROM is no substitute for real life , hands on experience , although when used as an adjunct to traditional teaching methods , it can enhance learning .
	manualset3
134623	5	406397	13	NULL	NULL	0	NULL	hands on experience	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that the CD-ROM is no substitute for real life , hands on experience , although when used as an adjunct to traditional teaching methods , it can enhance learning .
	manualset3
134624	6	406397	13	NULL	NULL	0	NULL	adjunct	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that the CD-ROM is no substitute for real life , hands on experience , although when used as an adjunct to traditional teaching methods , it can enhance learning .
	manualset3
134625	7	406397	13	NULL	NULL	0	NULL	traditional teaching methods	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that the CD-ROM is no substitute for real life , hands on experience , although when used as an adjunct to traditional teaching methods , it can enhance learning .
	manualset3
134626	8	406397	13	NULL	NULL	0	NULL	learning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that the CD-ROM is no substitute for real life , hands on experience , although when used as an adjunct to traditional teaching methods , it can enhance learning .
	manualset3
134627	1	406398	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results support the hypothesis that calcium is required for nicotine-induced neuroprotection in isolated pig RGCs .
	manualset3
134628	2	406398	13	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Results support the hypothesis that calcium is required for nicotine-induced neuroprotection in isolated pig RGCs .
	manualset3
134629	3	406398	13	NULL	NULL	0	NULL	calcium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Results support the hypothesis that calcium is required for nicotine-induced neuroprotection in isolated pig RGCs .
	manualset3
134630	4	406398	13	NULL	NULL	NULL	NULL	nicotine-induced neuroprotection	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Results support the hypothesis that calcium is required for nicotine-induced neuroprotection in isolated pig RGCs .
	manualset3
134631	5	406398	13	NULL	NULL	0	NULL	pig RGCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Results support the hypothesis that calcium is required for nicotine-induced neuroprotection in isolated pig RGCs .
	manualset3
134632	1	406399	13	NULL	NULL	NULL	NULL	Results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Results vary considerably probably as the profile of the surgical population changes .
	manualset3
134633	2	406399	13	NULL	NULL	0	NULL	profile	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results vary considerably probably as the profile of the surgical population changes .
	manualset3
134634	3	406399	13	NULL	NULL	0	NULL	surgical population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results vary considerably probably as the profile of the surgical population changes .
	manualset3
134636	1	406400	13	NULL	NULL	0	NULL	Results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Results were in well agreement with the macrocyclic size and cation radii relationships .
	manualset3
134637	2	406400	13	NULL	NULL	0	NULL	agreement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results were in well agreement with the macrocyclic size and cation radii relationships .
	manualset3
134638	3	406400	13	NULL	NULL	0	NULL	macrocyclic size	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Results were in well agreement with the macrocyclic size and cation radii relationships .
	manualset3
134639	4	406400	13	NULL	NULL	0	NULL	cation radii relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Results were in well agreement with the macrocyclic size and cation radii relationships .
	manualset3
134640	1	406401	13	NULL	NULL	0	NULL	Results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results were satisfactory although the most evident benefits were obtained with the first schedule , namely when treatment was commenced two days prior to operation .
	manualset3
134641	2	406401	13	NULL	NULL	0	NULL	benefits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results were satisfactory although the most evident benefits were obtained with the first schedule , namely when treatment was commenced two days prior to operation .
	manualset3
134642	3	406401	13	NULL	NULL	0	NULL	schedule	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results were satisfactory although the most evident benefits were obtained with the first schedule , namely when treatment was commenced two days prior to operation .
	manualset3
134643	4	406401	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Results were satisfactory although the most evident benefits were obtained with the first schedule , namely when treatment was commenced two days prior to operation .
	manualset3
134644	5	406401	13	NULL	NULL	0	NULL	two days 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Results were satisfactory although the most evident benefits were obtained with the first schedule , namely when treatment was commenced two days prior to operation .
	manualset3
134645	6	406401	13	NULL	NULL	0	NULL	operation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Results were satisfactory although the most evident benefits were obtained with the first schedule , namely when treatment was commenced two days prior to operation .
	manualset3
134646	1	406402	13	NULL	NULL	0	NULL	long-acting antihistamine-sympathomimetic combination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A new , long-acting antihistamine-sympathomimetic combination for the management of nasal congestion .
	manualset3
134647	2	406402	13	NULL	NULL	0	NULL	management 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A new , long-acting antihistamine-sympathomimetic combination for the management of nasal congestion .
	manualset3
134648	3	406402	13	NULL	NULL	0	NULL	nasal congestion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A new , long-acting antihistamine-sympathomimetic combination for the management of nasal congestion .
	manualset3
134649	1	406403	13	NULL	NULL	0	NULL	Results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results will have an important contribution to the estimation of childhood obesity , prediction of minimal weight in the athletic population and estimates of growth rate of fat and fat-free body mass. .
	manualset3
134650	2	406403	13	NULL	NULL	0	NULL	contribution	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results will have an important contribution to the estimation of childhood obesity , prediction of minimal weight in the athletic population and estimates of growth rate of fat and fat-free body mass. .
	manualset3
134651	3	406403	13	NULL	NULL	0	NULL	estimation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results will have an important contribution to the estimation of childhood obesity , prediction of minimal weight in the athletic population and estimates of growth rate of fat and fat-free body mass. .
	manualset3
134652	4	406403	13	NULL	NULL	0	NULL	childhood obesity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results will have an important contribution to the estimation of childhood obesity , prediction of minimal weight in the athletic population and estimates of growth rate of fat and fat-free body mass. .
	manualset3
134653	5	406403	13	NULL	NULL	0	NULL	prediction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results will have an important contribution to the estimation of childhood obesity , prediction of minimal weight in the athletic population and estimates of growth rate of fat and fat-free body mass. .
	manualset3
134654	6	406403	13	NULL	NULL	0	NULL	minimal weight	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results will have an important contribution to the estimation of childhood obesity , prediction of minimal weight in the athletic population and estimates of growth rate of fat and fat-free body mass. .
	manualset3
134655	7	406403	13	NULL	NULL	0	NULL	athletic population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results will have an important contribution to the estimation of childhood obesity , prediction of minimal weight in the athletic population and estimates of growth rate of fat and fat-free body mass. .
	manualset3
134656	8	406403	13	NULL	NULL	0	NULL	estimates	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results will have an important contribution to the estimation of childhood obesity , prediction of minimal weight in the athletic population and estimates of growth rate of fat and fat-free body mass. .
	manualset3
134657	9	406403	13	NULL	NULL	0	NULL	 growth rate of fat	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results will have an important contribution to the estimation of childhood obesity , prediction of minimal weight in the athletic population and estimates of growth rate of fat and fat-free body mass. .
	manualset3
134658	10	406403	13	NULL	NULL	0	NULL	fat-free body mass	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results will have an important contribution to the estimation of childhood obesity , prediction of minimal weight in the athletic population and estimates of growth rate of fat and fat-free body mass. .
	manualset3
134659	1	406404	13	NULL	NULL	0	NULL	Resuscitation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Resuscitation of the brain after cardiac arrest , the most frequent reason for global cerebral ischemia under clinical conditions , depends critically on the reversal of disturbances of water and ion homeostasis .
	manualset3
134660	2	406404	13	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Resuscitation of the brain after cardiac arrest , the most frequent reason for global cerebral ischemia under clinical conditions , depends critically on the reversal of disturbances of water and ion homeostasis .
	manualset3
134661	3	406404	13	NULL	NULL	0	NULL	cardiac arrest	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Resuscitation of the brain after cardiac arrest , the most frequent reason for global cerebral ischemia under clinical conditions , depends critically on the reversal of disturbances of water and ion homeostasis .
	manualset3
134662	4	406404	13	NULL	NULL	0	NULL	reason	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Resuscitation of the brain after cardiac arrest , the most frequent reason for global cerebral ischemia under clinical conditions , depends critically on the reversal of disturbances of water and ion homeostasis .
	manualset3
134663	5	406404	13	NULL	NULL	0	NULL	global cerebral ischemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Resuscitation of the brain after cardiac arrest , the most frequent reason for global cerebral ischemia under clinical conditions , depends critically on the reversal of disturbances of water and ion homeostasis .
	manualset3
134664	6	406404	13	NULL	NULL	0	NULL	clinical conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Resuscitation of the brain after cardiac arrest , the most frequent reason for global cerebral ischemia under clinical conditions , depends critically on the reversal of disturbances of water and ion homeostasis .
	manualset3
134665	7	406404	13	NULL	NULL	0	NULL	reversal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Resuscitation of the brain after cardiac arrest , the most frequent reason for global cerebral ischemia under clinical conditions , depends critically on the reversal of disturbances of water and ion homeostasis .
	manualset3
134666	8	406404	13	NULL	NULL	0	NULL	disturbances 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Resuscitation of the brain after cardiac arrest , the most frequent reason for global cerebral ischemia under clinical conditions , depends critically on the reversal of disturbances of water and ion homeostasis .
	manualset3
134667	9	406404	13	NULL	NULL	0	NULL	water homeostasis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Resuscitation of the brain after cardiac arrest , the most frequent reason for global cerebral ischemia under clinical conditions , depends critically on the reversal of disturbances of water and ion homeostasis .
	manualset3
134668	10	406404	13	NULL	NULL	0	NULL	ion homeostasis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Resuscitation of the brain after cardiac arrest , the most frequent reason for global cerebral ischemia under clinical conditions , depends critically on the reversal of disturbances of water and ion homeostasis .
	manualset3
134669	1	406405	13	NULL	NULL	0	NULL	Resveratrol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Resveratrol decreases the levels of miR-155 by upregulating miR-663 , a microRNA targeting JunB and JunD .
	manualset3
134670	2	406405	13	NULL	NULL	0	NULL	levels 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Resveratrol decreases the levels of miR-155 by upregulating miR-663 , a microRNA targeting JunB and JunD .
	manualset3
134671	3	406405	13	NULL	NULL	0	NULL	miR-155 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Resveratrol decreases the levels of miR-155 by upregulating miR-663 , a microRNA targeting JunB and JunD .
	manualset3
134672	4	406405	13	NULL	NULL	0	NULL	miR-663	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Resveratrol decreases the levels of miR-155 by upregulating miR-663 , a microRNA targeting JunB and JunD .
	manualset3
134673	5	406405	13	NULL	NULL	0	NULL	microRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Resveratrol decreases the levels of miR-155 by upregulating miR-663 , a microRNA targeting JunB and JunD .
	manualset3
134674	6	406405	13	NULL	NULL	0	NULL	JunB	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Resveratrol decreases the levels of miR-155 by upregulating miR-663 , a microRNA targeting JunB and JunD .
	manualset3
134675	7	406405	13	NULL	NULL	0	NULL	JunD	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Resveratrol decreases the levels of miR-155 by upregulating miR-663 , a microRNA targeting JunB and JunD .
	manualset3
134676	1	406406	13	NULL	NULL	0	NULL	Reticulocalbin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Reticulocalbin and ERC-55 localize to the ER due to a C-terminal HDEL retrieval signal .
	manualset3
134677	2	406406	13	NULL	NULL	0	NULL	ERC-55	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reticulocalbin and ERC-55 localize to the ER due to a C-terminal HDEL retrieval signal .
	manualset3
134678	3	406406	13	NULL	NULL	0	NULL	ER 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Reticulocalbin and ERC-55 localize to the ER due to a C-terminal HDEL retrieval signal .
	manualset3
134679	4	406406	13	NULL	NULL	0	NULL	C-terminal HDEL retrieval signal	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reticulocalbin and ERC-55 localize to the ER due to a C-terminal HDEL retrieval signal .
	manualset3
134680	1	406407	13	NULL	NULL	0	NULL	Retinal pigment epithelium ( RPE ) pigmentation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinal pigment epithelium ( RPE ) pigmentation and thickening in the central macula after macular edema resolution in central retinal vein occlusion ( CRVO ) .
	manualset3
134681	2	406407	13	NULL	NULL	0	NULL	central macula	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinal pigment epithelium ( RPE ) pigmentation and thickening in the central macula after macular edema resolution in central retinal vein occlusion ( CRVO ) .
	manualset3
134682	3	406407	13	NULL	NULL	0	NULL	macular edema resolution	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinal pigment epithelium ( RPE ) pigmentation and thickening in the central macula after macular edema resolution in central retinal vein occlusion ( CRVO ) .
	manualset3
134683	4	406407	13	NULL	NULL	0	NULL	central retinal vein occlusion ( CRVO ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinal pigment epithelium ( RPE ) pigmentation and thickening in the central macula after macular edema resolution in central retinal vein occlusion ( CRVO ) .
	manualset3
134684	1	406408	13	NULL	NULL	0	NULL	Retinal venous oxygen saturation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinal venous oxygen saturation and cardiac output during controlled hemorrhage and resuscitation .
	manualset3
134685	2	406408	13	NULL	NULL	0	NULL	cardiac output 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinal venous oxygen saturation and cardiac output during controlled hemorrhage and resuscitation .
	manualset3
134686	3	406408	13	NULL	NULL	0	NULL	hemorrhage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinal venous oxygen saturation and cardiac output during controlled hemorrhage and resuscitation .
	manualset3
134687	4	406408	13	NULL	NULL	0	NULL	resuscitation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinal venous oxygen saturation and cardiac output during controlled hemorrhage and resuscitation .
	manualset3
134688	1	406409	13	NULL	NULL	0	NULL	Retinoic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinoic acid upregulates preadipocyte genes to block adipogenesis and suppress diet-induced obesity .
	manualset3
134689	2	406409	13	NULL	NULL	0	NULL	preadipocyte genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinoic acid upregulates preadipocyte genes to block adipogenesis and suppress diet-induced obesity .
	manualset3
134690	3	406409	13	NULL	NULL	0	NULL	adipogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinoic acid upregulates preadipocyte genes to block adipogenesis and suppress diet-induced obesity .
	manualset3
134691	4	406409	13	NULL	NULL	0	NULL	obesity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinoic acid upregulates preadipocyte genes to block adipogenesis and suppress diet-induced obesity .
	manualset3
134692	1	406410	13	NULL	NULL	0	NULL	Retinoid X receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinoid X receptor and retinoic acid response in the marine sponge Suberites domuncula .
	manualset3
134693	2	406410	13	NULL	NULL	0	NULL	retinoic acid response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinoid X receptor and retinoic acid response in the marine sponge Suberites domuncula .
	manualset3
134694	3	406410	13	NULL	NULL	0	NULL	marine sponge Suberites domuncula	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinoid X receptor and retinoic acid response in the marine sponge Suberites domuncula .
	manualset3
134695	1	406411	13	NULL	NULL	0	NULL	branches	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinotopically appropriate branches and synapses may be stabilized because the normally correlated firing of neighboring ganglion cells could cause summation of their postsynaptic responses , making them more effective .
	manualset3
134696	2	406411	13	NULL	NULL	0	NULL	synapses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinotopically appropriate branches and synapses may be stabilized because the normally correlated firing of neighboring ganglion cells could cause summation of their postsynaptic responses , making them more effective .
	manualset3
134697	3	406411	13	NULL	NULL	0	NULL	firing 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinotopically appropriate branches and synapses may be stabilized because the normally correlated firing of neighboring ganglion cells could cause summation of their postsynaptic responses , making them more effective .
	manualset3
134698	4	406411	13	NULL	NULL	0	NULL	ganglion cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinotopically appropriate branches and synapses may be stabilized because the normally correlated firing of neighboring ganglion cells could cause summation of their postsynaptic responses , making them more effective .
	manualset3
134699	5	406411	13	NULL	NULL	0	NULL	summation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinotopically appropriate branches and synapses may be stabilized because the normally correlated firing of neighboring ganglion cells could cause summation of their postsynaptic responses , making them more effective .
	manualset3
134700	6	406411	13	NULL	NULL	0	NULL	postsynaptic responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinotopically appropriate branches and synapses may be stabilized because the normally correlated firing of neighboring ganglion cells could cause summation of their postsynaptic responses , making them more effective .
	manualset3
134701	1	406412	13	NULL	NULL	0	NULL	Retinyl palmitate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinyl palmitate was present in rabbit lacrimal gland at 51.0 + / - 10.1 ng/g tissue .
	manualset3
134702	2	406412	13	NULL	NULL	0	NULL	rabbit lacrimal gland	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinyl palmitate was present in rabbit lacrimal gland at 51.0 + / - 10.1 ng/g tissue .
	manualset3
134703	3	406412	13	NULL	NULL	0	NULL	51.0 + / - 10.1 ng/g tissue	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinyl palmitate was present in rabbit lacrimal gland at 51.0 + / - 10.1 ng/g tissue .
	manualset3
134704	1	406413	13	NULL	NULL	0	NULL	Retraction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Retraction : Facile palladium-catalyzed arylation of heterocycles and nonactivated arenes with aryl chlorides .
	manualset3
134705	2	406413	13	NULL	NULL	0	NULL	palladium-catalyzed arylation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Retraction : Facile palladium-catalyzed arylation of heterocycles and nonactivated arenes with aryl chlorides .
	manualset3
134706	3	406413	13	NULL	NULL	0	NULL	heterocycles	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Retraction : Facile palladium-catalyzed arylation of heterocycles and nonactivated arenes with aryl chlorides .
	manualset3
134707	4	406413	13	NULL	NULL	0	NULL	arenes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Retraction : Facile palladium-catalyzed arylation of heterocycles and nonactivated arenes with aryl chlorides .
	manualset3
134708	5	406413	13	NULL	NULL	0	NULL	aryl chlorides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Retraction : Facile palladium-catalyzed arylation of heterocycles and nonactivated arenes with aryl chlorides .
	manualset3
134709	1	406414	13	NULL	NULL	0	NULL	Retraction notice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Retraction notice to `` Validation and application of a high-performance liquid chromatographic-based assay for determination of the inosine 5 ' - monophosphate dehydrogenase activity in erythrocytes . ''
	manualset3
134710	2	406414	13	NULL	NULL	0	NULL	Validation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Retraction notice to `` Validation and application of a high-performance liquid chromatographic-based assay for determination of the inosine 5 ' - monophosphate dehydrogenase activity in erythrocytes . ''
	manualset3
134711	3	406414	13	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Retraction notice to `` Validation and application of a high-performance liquid chromatographic-based assay for determination of the inosine 5 ' - monophosphate dehydrogenase activity in erythrocytes . ''
	manualset3
134712	4	406414	13	NULL	NULL	0	NULL	high-performance liquid chromatographic-based assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Retraction notice to `` Validation and application of a high-performance liquid chromatographic-based assay for determination of the inosine 5 ' - monophosphate dehydrogenase activity in erythrocytes . ''
	manualset3
134713	5	406414	13	NULL	NULL	0	NULL	determination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Retraction notice to `` Validation and application of a high-performance liquid chromatographic-based assay for determination of the inosine 5 ' - monophosphate dehydrogenase activity in erythrocytes . ''
	manualset3
134714	6	406414	13	NULL	NULL	0	NULL	inosine 5 ' - monophosphate dehydrogenase activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Retraction notice to `` Validation and application of a high-performance liquid chromatographic-based assay for determination of the inosine 5 ' - monophosphate dehydrogenase activity in erythrocytes . ''
	manualset3
134715	7	406414	13	NULL	NULL	0	NULL	erythrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Retraction notice to `` Validation and application of a high-performance liquid chromatographic-based assay for determination of the inosine 5 ' - monophosphate dehydrogenase activity in erythrocytes . ''
	manualset3
134716	1	406415	13	NULL	NULL	0	NULL	Retrospective evaluation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Retrospective evaluation of treatment outcome in Japanese children with complete unilateral cleft lip and palate .
	manualset3
134717	2	406415	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Retrospective evaluation of treatment outcome in Japanese children with complete unilateral cleft lip and palate .
	manualset3
134718	3	406415	13	NULL	NULL	0	NULL	outcome 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Retrospective evaluation of treatment outcome in Japanese children with complete unilateral cleft lip and palate .
	manualset3
134719	4	406415	13	NULL	NULL	0	NULL	Japanese children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Retrospective evaluation of treatment outcome in Japanese children with complete unilateral cleft lip and palate .
	manualset3
134720	5	406415	13	NULL	NULL	NULL	NULL	complete unilateral cleft lip and palate 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Retrospective evaluation of treatment outcome in Japanese children with complete unilateral cleft lip and palate .
	manualset3
134722	1	406416	13	NULL	NULL	0	NULL	Retrotransposons	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Retrotransposons and their remnants often constitute more than 50 % of higher plant genomes .
	manualset3
134723	2	406416	13	NULL	NULL	0	NULL	remnants	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Retrotransposons and their remnants often constitute more than 50 % of higher plant genomes .
	manualset3
134724	3	406416	13	NULL	NULL	0	NULL	50 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Retrotransposons and their remnants often constitute more than 50 % of higher plant genomes .
	manualset3
134725	4	406416	13	NULL	NULL	0	NULL	higher plant genomes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Retrotransposons and their remnants often constitute more than 50 % of higher plant genomes .
	manualset3
134726	1	406417	13	NULL	NULL	0	NULL	Retroviral insertional activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Retroviral insertional activation of the Fli-3 locus in erythroleukemias encoding a cluster of microRNAs that convert Epo-induced differentiation to proliferation .
	manualset3
134727	2	406417	13	NULL	NULL	0	NULL	Fli-3 locus	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Retroviral insertional activation of the Fli-3 locus in erythroleukemias encoding a cluster of microRNAs that convert Epo-induced differentiation to proliferation .
	manualset3
134728	3	406417	13	NULL	NULL	0	NULL	erythroleukemias	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Retroviral insertional activation of the Fli-3 locus in erythroleukemias encoding a cluster of microRNAs that convert Epo-induced differentiation to proliferation .
	manualset3
134729	4	406417	13	NULL	NULL	0	NULL	cluster of microRNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Retroviral insertional activation of the Fli-3 locus in erythroleukemias encoding a cluster of microRNAs that convert Epo-induced differentiation to proliferation .
	manualset3
134730	5	406417	13	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Retroviral insertional activation of the Fli-3 locus in erythroleukemias encoding a cluster of microRNAs that convert Epo-induced differentiation to proliferation .
	manualset3
134731	6	406417	13	NULL	NULL	0	NULL	proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Retroviral insertional activation of the Fli-3 locus in erythroleukemias encoding a cluster of microRNAs that convert Epo-induced differentiation to proliferation .
	manualset3
134732	1	406418	13	NULL	NULL	NULL	NULL	Returns	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Returns from protein therapeutics are experiencing unprecedented growth : both their number and their economic dividend have increased by an order of magnitude in the last 10 years .
	manualset3
134733	2	406418	13	NULL	NULL	0	NULL	protein therapeutics	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Returns from protein therapeutics are experiencing unprecedented growth : both their number and their economic dividend have increased by an order of magnitude in the last 10 years .
	manualset3
134734	3	406418	13	NULL	NULL	0	NULL	growth	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Returns from protein therapeutics are experiencing unprecedented growth : both their number and their economic dividend have increased by an order of magnitude in the last 10 years .
	manualset3
134735	4	406418	13	NULL	NULL	0	NULL	number	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Returns from protein therapeutics are experiencing unprecedented growth : both their number and their economic dividend have increased by an order of magnitude in the last 10 years .
	manualset3
134736	5	406418	13	NULL	NULL	0	NULL	economic dividend	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Returns from protein therapeutics are experiencing unprecedented growth : both their number and their economic dividend have increased by an order of magnitude in the last 10 years .
	manualset3
134738	6	406418	13	NULL	NULL	0	NULL	order of magnitude 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Returns from protein therapeutics are experiencing unprecedented growth : both their number and their economic dividend have increased by an order of magnitude in the last 10 years .
	manualset3
134739	7	406418	13	NULL	NULL	0	NULL	last 10 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Returns from protein therapeutics are experiencing unprecedented growth : both their number and their economic dividend have increased by an order of magnitude in the last 10 years .
	manualset3
134740	1	406419	13	NULL	NULL	0	NULL	Reusability investigation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reusability investigation showed that more than 60 % of the initial activity was remained after six reuses of immobilized enzyme on Unc-LDH-CO ( 3 ) and C-LDH-CO ( 3 ) .
	manualset3
134741	2	406419	13	NULL	NULL	0	NULL	60 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Reusability investigation showed that more than 60 % of the initial activity was remained after six reuses of immobilized enzyme on Unc-LDH-CO ( 3 ) and C-LDH-CO ( 3 ) .
	manualset3
134742	3	406419	13	NULL	NULL	NULL	NULL	initial activity	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Reusability investigation showed that more than 60 % of the initial activity was remained after six reuses of immobilized enzyme on Unc-LDH-CO ( 3 ) and C-LDH-CO ( 3 ) .
	manualset3
134743	4	406419	13	NULL	NULL	NULL	NULL	six reuses	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Reusability investigation showed that more than 60 % of the initial activity was remained after six reuses of immobilized enzyme on Unc-LDH-CO ( 3 ) and C-LDH-CO ( 3 ) .
	manualset3
134744	5	406419	13	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Reusability investigation showed that more than 60 % of the initial activity was remained after six reuses of immobilized enzyme on Unc-LDH-CO ( 3 ) and C-LDH-CO ( 3 ) .
	manualset3
134745	6	406419	13	NULL	NULL	0	NULL	Unc-LDH-CO ( 3 ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Reusability investigation showed that more than 60 % of the initial activity was remained after six reuses of immobilized enzyme on Unc-LDH-CO ( 3 ) and C-LDH-CO ( 3 ) .
	manualset3
134746	7	406419	13	NULL	NULL	0	NULL	C-LDH-CO ( 3 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Reusability investigation showed that more than 60 % of the initial activity was remained after six reuses of immobilized enzyme on Unc-LDH-CO ( 3 ) and C-LDH-CO ( 3 ) .
	manualset3
134747	1	406420	13	NULL	NULL	0	NULL	Rev. E 78 , 031120 ( 2008 ) 	Journal												NULL		0	NULL	NULL	NULL	NULL	NULL	Rev. E 78 , 031120 ( 2008 ) ) , where the connection between the occurrence of energetic instability and stochastic multiresonance is established .
	manualset3
134748	2	406420	13	NULL	NULL	0	NULL	connection	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Rev. E 78 , 031120 ( 2008 ) ) , where the connection between the occurrence of energetic instability and stochastic multiresonance is established .
	manualset3
134749	3	406420	13	NULL	NULL	0	NULL	occurrence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rev. E 78 , 031120 ( 2008 ) ) , where the connection between the occurrence of energetic instability and stochastic multiresonance is established .
	manualset3
134750	4	406420	13	NULL	NULL	0	NULL	energetic instability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rev. E 78 , 031120 ( 2008 ) ) , where the connection between the occurrence of energetic instability and stochastic multiresonance is established .
	manualset3
134751	5	406420	13	NULL	NULL	0	NULL	stochastic multiresonance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rev. E 78 , 031120 ( 2008 ) ) , where the connection between the occurrence of energetic instability and stochastic multiresonance is established .
	manualset3
134752	1	406421	13	NULL	NULL	0	NULL	BAC vector	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A new BAC vector that allows color-based positive screening to identify transformants with inserts has increased BAC cloning efficiency .
	manualset3
134753	2	406421	13	NULL	NULL	0	NULL	color-based positive screening	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new BAC vector that allows color-based positive screening to identify transformants with inserts has increased BAC cloning efficiency .
	manualset3
134754	3	406421	13	NULL	NULL	0	NULL	transformants	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A new BAC vector that allows color-based positive screening to identify transformants with inserts has increased BAC cloning efficiency .
	manualset3
134755	4	406421	13	NULL	NULL	0	NULL	inserts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A new BAC vector that allows color-based positive screening to identify transformants with inserts has increased BAC cloning efficiency .
	manualset3
134756	5	406421	13	NULL	NULL	0	NULL	BAC cloning efficiency	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A new BAC vector that allows color-based positive screening to identify transformants with inserts has increased BAC cloning efficiency .
	manualset3
134757	1	406422	13	NULL	NULL	0	NULL	Revenues	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Revenues drop , health spending rises : what 's a state to do ?
	manualset3
134758	2	406422	13	NULL	NULL	0	NULL	health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Revenues drop , health spending rises : what 's a state to do ?
	manualset3
134759	3	406422	13	NULL	NULL	0	NULL	rises	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Revenues drop , health spending rises : what 's a state to do ?
	manualset3
134760	4	406422	13	NULL	NULL	0	NULL	state	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Revenues drop , health spending rises : what 's a state to do ?
	manualset3
134761	1	406423	13	NULL	NULL	0	NULL	Reversan	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversan , the lead compound of this class , increased the efficacy of both vincristine and etoposide in murine models of neuroblastoma ( syngeneic and human xenografts ) .
	manualset3
134762	2	406423	13	NULL	NULL	0	NULL	lead compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversan , the lead compound of this class , increased the efficacy of both vincristine and etoposide in murine models of neuroblastoma ( syngeneic and human xenografts ) .
	manualset3
134763	3	406423	13	NULL	NULL	0	NULL	class	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversan , the lead compound of this class , increased the efficacy of both vincristine and etoposide in murine models of neuroblastoma ( syngeneic and human xenografts ) .
	manualset3
134764	4	406423	13	NULL	NULL	0	NULL	efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversan , the lead compound of this class , increased the efficacy of both vincristine and etoposide in murine models of neuroblastoma ( syngeneic and human xenografts ) .
	manualset3
134765	5	406423	13	NULL	NULL	0	NULL	vincristine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversan , the lead compound of this class , increased the efficacy of both vincristine and etoposide in murine models of neuroblastoma ( syngeneic and human xenografts ) .
	manualset3
134766	6	406423	13	NULL	NULL	0	NULL	etoposide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversan , the lead compound of this class , increased the efficacy of both vincristine and etoposide in murine models of neuroblastoma ( syngeneic and human xenografts ) .
	manualset3
134767	7	406423	13	NULL	NULL	0	NULL	murine models 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversan , the lead compound of this class , increased the efficacy of both vincristine and etoposide in murine models of neuroblastoma ( syngeneic and human xenografts ) .
	manualset3
134768	8	406423	13	NULL	NULL	0	NULL	neuroblastoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversan , the lead compound of this class , increased the efficacy of both vincristine and etoposide in murine models of neuroblastoma ( syngeneic and human xenografts ) .
	manualset3
134769	9	406423	13	NULL	NULL	0	NULL	human xenografts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversan , the lead compound of this class , increased the efficacy of both vincristine and etoposide in murine models of neuroblastoma ( syngeneic and human xenografts ) .
	manualset3
134770	1	406424	13	NULL	NULL	0	NULL	Reversibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversibility of the effects of chronic paternal exposure to cyclophosphamide on pregnancy outcome in rats .
	manualset3
134771	2	406424	13	NULL	NULL	0	NULL	effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversibility of the effects of chronic paternal exposure to cyclophosphamide on pregnancy outcome in rats .
	manualset3
134772	3	406424	13	NULL	NULL	0	NULL	chronic paternal exposure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversibility of the effects of chronic paternal exposure to cyclophosphamide on pregnancy outcome in rats .
	manualset3
134773	4	406424	13	NULL	NULL	0	NULL	cyclophosphamide 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversibility of the effects of chronic paternal exposure to cyclophosphamide on pregnancy outcome in rats .
	manualset3
134774	5	406424	13	NULL	NULL	0	NULL	pregnancy outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversibility of the effects of chronic paternal exposure to cyclophosphamide on pregnancy outcome in rats .
	manualset3
134775	6	406424	13	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversibility of the effects of chronic paternal exposure to cyclophosphamide on pregnancy outcome in rats .
	manualset3
134776	1	406425	13	NULL	NULL	0	NULL	Reversible abnormal regional contraction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversible abnormal regional contraction of the myocardium was demonstrated and correlated with a reversible perfusion defect on subsequent thallium myocardial perfusion imaging and a blocked artery at coronary angiography .
	manualset3
134777	2	406425	13	NULL	NULL	0	NULL	myocardium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversible abnormal regional contraction of the myocardium was demonstrated and correlated with a reversible perfusion defect on subsequent thallium myocardial perfusion imaging and a blocked artery at coronary angiography .
	manualset3
134778	3	406425	13	NULL	NULL	0	NULL	reversible perfusion defect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversible abnormal regional contraction of the myocardium was demonstrated and correlated with a reversible perfusion defect on subsequent thallium myocardial perfusion imaging and a blocked artery at coronary angiography .
	manualset3
134779	4	406425	13	NULL	NULL	0	NULL	thallium myocardial perfusion imaging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversible abnormal regional contraction of the myocardium was demonstrated and correlated with a reversible perfusion defect on subsequent thallium myocardial perfusion imaging and a blocked artery at coronary angiography .
	manualset3
134780	5	406425	13	NULL	NULL	0	NULL	artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversible abnormal regional contraction of the myocardium was demonstrated and correlated with a reversible perfusion defect on subsequent thallium myocardial perfusion imaging and a blocked artery at coronary angiography .
	manualset3
134781	6	406425	13	NULL	NULL	0	NULL	coronary angiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversible abnormal regional contraction of the myocardium was demonstrated and correlated with a reversible perfusion defect on subsequent thallium myocardial perfusion imaging and a blocked artery at coronary angiography .
	manualset3
134782	1	406426	13	NULL	NULL	0	NULL	Reversible interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversible and irreversible interactions between lysozyme and soft contact lens surfaces .
	manualset3
134783	2	406426	13	NULL	NULL	0	NULL	irreversible interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversible and irreversible interactions between lysozyme and soft contact lens surfaces .
	manualset3
134784	3	406426	13	NULL	NULL	0	NULL	 lysozyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversible and irreversible interactions between lysozyme and soft contact lens surfaces .
	manualset3
134785	4	406426	13	NULL	NULL	0	NULL	soft contact lens surfaces	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversible and irreversible interactions between lysozyme and soft contact lens surfaces .
	manualset3
134786	1	406427	13	NULL	NULL	0	NULL	Reversible perfusion defects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversible perfusion defects within infarct related artery territory occurred with similar frequency in both treatment groups ( rTPA 7 , placebo 8 ) .
	manualset3
134787	2	406427	13	NULL	NULL	0	NULL	infarct related artery territory 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversible perfusion defects within infarct related artery territory occurred with similar frequency in both treatment groups ( rTPA 7 , placebo 8 ) .
	manualset3
134788	3	406427	13	NULL	NULL	0	NULL	frequency	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversible perfusion defects within infarct related artery territory occurred with similar frequency in both treatment groups ( rTPA 7 , placebo 8 ) .
	manualset3
134789	4	406427	13	NULL	NULL	0	NULL	treatment groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversible perfusion defects within infarct related artery territory occurred with similar frequency in both treatment groups ( rTPA 7 , placebo 8 ) .
	manualset3
134790	5	406427	13	NULL	NULL	0	NULL	 rTPA 7	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversible perfusion defects within infarct related artery territory occurred with similar frequency in both treatment groups ( rTPA 7 , placebo 8 ) .
	manualset3
134791	6	406427	13	NULL	NULL	0	NULL	placebo 8 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversible perfusion defects within infarct related artery territory occurred with similar frequency in both treatment groups ( rTPA 7 , placebo 8 ) .
	manualset3
134792	1	406428	13	NULL	NULL	0	NULL	Reversion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversion to a non-aggressive phenotype seems possible and gives therapeutic hope .
	manualset3
134793	2	406428	13	NULL	NULL	0	NULL	non-aggressive phenotype	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversion to a non-aggressive phenotype seems possible and gives therapeutic hope .
	manualset3
134794	3	406428	13	NULL	NULL	0	NULL	therapeutic hope	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversion to a non-aggressive phenotype seems possible and gives therapeutic hope .
	manualset3
134795	1	406429	13	NULL	NULL	0	NULL	Care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Care of hip and knee arthroses must be equal ) .
	manualset3
134796	2	406429	13	NULL	NULL	0	NULL	hip arthroses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Care of hip and knee arthroses must be equal ) .
	manualset3
134797	3	406429	13	NULL	NULL	0	NULL	knee arthroses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Care of hip and knee arthroses must be equal ) .
	manualset3
134798	1	406430	13	NULL	NULL	0	NULL	Review	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Review : Insufficient evidence exists to determine the benefits and risks of statins for acute stroke or TIA .
	manualset3
134799	2	406430	13	NULL	NULL	0	NULL	Insufficient evidence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Review : Insufficient evidence exists to determine the benefits and risks of statins for acute stroke or TIA .
	manualset3
134800	3	406430	13	NULL	NULL	0	NULL	benefits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Review : Insufficient evidence exists to determine the benefits and risks of statins for acute stroke or TIA .
	manualset3
134801	4	406430	13	NULL	NULL	0	NULL	risks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Review : Insufficient evidence exists to determine the benefits and risks of statins for acute stroke or TIA .
	manualset3
134802	5	406430	13	NULL	NULL	0	NULL	statins	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Review : Insufficient evidence exists to determine the benefits and risks of statins for acute stroke or TIA .
	manualset3
134803	6	406430	13	NULL	NULL	0	NULL	acute stroke	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Review : Insufficient evidence exists to determine the benefits and risks of statins for acute stroke or TIA .
	manualset3
134804	7	406430	13	NULL	NULL	0	NULL	TIA	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Review : Insufficient evidence exists to determine the benefits and risks of statins for acute stroke or TIA .
	manualset3
134807	1	406431	13	NULL	NULL	0	NULL	Review 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Review : response to SSRIs in unipolar depression occurs in the first week of treatment .
	manualset3
134808	2	406431	13	NULL	NULL	0	NULL	response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Review : response to SSRIs in unipolar depression occurs in the first week of treatment .
	manualset3
134809	3	406431	13	NULL	NULL	0	NULL	SSRIs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Review : response to SSRIs in unipolar depression occurs in the first week of treatment .
	manualset3
134810	4	406431	13	NULL	NULL	0	NULL	unipolar depression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Review : response to SSRIs in unipolar depression occurs in the first week of treatment .
	manualset3
134811	5	406431	13	NULL	NULL	0	NULL	week	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Review : response to SSRIs in unipolar depression occurs in the first week of treatment .
	manualset3
134812	6	406431	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Review : response to SSRIs in unipolar depression occurs in the first week of treatment .
	manualset3
134898	1	406432	13	NULL	NULL	0	NULL	Review 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of National League for Nursing and Center for Human Caring videotape `` a guide to applying the art and science of human caring : a consultation with Jean Watson and colleagues , '' Parts 1 and 2 .
	manualset3
134899	2	406432	13	NULL	NULL	0	NULL	National League for Nursing	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of National League for Nursing and Center for Human Caring videotape `` a guide to applying the art and science of human caring : a consultation with Jean Watson and colleagues , '' Parts 1 and 2 .
	manualset3
134900	3	406432	13	NULL	NULL	0	NULL	Center for Human Caring	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of National League for Nursing and Center for Human Caring videotape `` a guide to applying the art and science of human caring : a consultation with Jean Watson and colleagues , '' Parts 1 and 2 .
	manualset3
134901	4	406432	13	NULL	NULL	0	NULL	videotape	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of National League for Nursing and Center for Human Caring videotape `` a guide to applying the art and science of human caring : a consultation with Jean Watson and colleagues , '' Parts 1 and 2 .
	manualset3
134902	5	406432	13	NULL	NULL	0	NULL	guide	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of National League for Nursing and Center for Human Caring videotape `` a guide to applying the art and science of human caring : a consultation with Jean Watson and colleagues , '' Parts 1 and 2 .
	manualset3
134903	6	406432	13	NULL	NULL	0	NULL	art 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of National League for Nursing and Center for Human Caring videotape `` a guide to applying the art and science of human caring : a consultation with Jean Watson and colleagues , '' Parts 1 and 2 .
	manualset3
134904	7	406432	13	NULL	NULL	0	NULL	science	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of National League for Nursing and Center for Human Caring videotape `` a guide to applying the art and science of human caring : a consultation with Jean Watson and colleagues , '' Parts 1 and 2 .
	manualset3
134905	8	406432	13	NULL	NULL	0	NULL	human caring 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of National League for Nursing and Center for Human Caring videotape `` a guide to applying the art and science of human caring : a consultation with Jean Watson and colleagues , '' Parts 1 and 2 .
	manualset3
134906	9	406432	13	NULL	NULL	0	NULL	consultation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of National League for Nursing and Center for Human Caring videotape `` a guide to applying the art and science of human caring : a consultation with Jean Watson and colleagues , '' Parts 1 and 2 .
	manualset3
134907	10	406432	13	NULL	NULL	0	NULL	Jean Watson	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of National League for Nursing and Center for Human Caring videotape `` a guide to applying the art and science of human caring : a consultation with Jean Watson and colleagues , '' Parts 1 and 2 .
	manualset3
134908	11	406432	13	NULL	NULL	0	NULL	colleagues	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of National League for Nursing and Center for Human Caring videotape `` a guide to applying the art and science of human caring : a consultation with Jean Watson and colleagues , '' Parts 1 and 2 .
	manualset3
134909	12	406432	13	NULL	NULL	0	NULL	Parts 1	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of National League for Nursing and Center for Human Caring videotape `` a guide to applying the art and science of human caring : a consultation with Jean Watson and colleagues , '' Parts 1 and 2 .
	manualset3
134910	13	406432	13	NULL	NULL	0	NULL	Parts 2	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of National League for Nursing and Center for Human Caring videotape `` a guide to applying the art and science of human caring : a consultation with Jean Watson and colleagues , '' Parts 1 and 2 .
	manualset3
134911	1	406433	13	NULL	NULL	0	NULL	Review	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of the literature indicated that the interface between the rubber boot sole and rubber matting was associated with a very high coefficient of friction , probably causing excessive torque at the knee .
	manualset3
134912	2	406433	13	NULL	NULL	0	NULL	literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of the literature indicated that the interface between the rubber boot sole and rubber matting was associated with a very high coefficient of friction , probably causing excessive torque at the knee .
	manualset3
134913	3	406433	13	NULL	NULL	0	NULL	interface	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of the literature indicated that the interface between the rubber boot sole and rubber matting was associated with a very high coefficient of friction , probably causing excessive torque at the knee .
	manualset3
134914	4	406433	13	NULL	NULL	0	NULL	rubber boot sole	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of the literature indicated that the interface between the rubber boot sole and rubber matting was associated with a very high coefficient of friction , probably causing excessive torque at the knee .
	manualset3
134915	5	406433	13	NULL	NULL	0	NULL	rubber matting	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of the literature indicated that the interface between the rubber boot sole and rubber matting was associated with a very high coefficient of friction , probably causing excessive torque at the knee .
	manualset3
134916	6	406433	13	NULL	NULL	0	NULL	coefficient of friction 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of the literature indicated that the interface between the rubber boot sole and rubber matting was associated with a very high coefficient of friction , probably causing excessive torque at the knee .
	manualset3
134917	7	406433	13	NULL	NULL	0	NULL	torque	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of the literature indicated that the interface between the rubber boot sole and rubber matting was associated with a very high coefficient of friction , probably causing excessive torque at the knee .
	manualset3
134918	8	406433	13	NULL	NULL	0	NULL	knee	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of the literature indicated that the interface between the rubber boot sole and rubber matting was associated with a very high coefficient of friction , probably causing excessive torque at the knee .
	manualset3
134919	1	406434	13	NULL	NULL	0	NULL	Review 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of the literature revealed that the quality of dying and death construct is multidimensional , with 7 broad domains : physical experience , psychological experience , social experience , spiritual or existential experience , the nature of health care , life closure and death preparation , and the circumstances of death .
	manualset3
134920	2	406434	13	NULL	NULL	0	NULL	literature 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of the literature revealed that the quality of dying and death construct is multidimensional , with 7 broad domains : physical experience , psychological experience , social experience , spiritual or existential experience , the nature of health care , life closure and death preparation , and the circumstances of death .
	manualset3
134921	3	406434	13	NULL	NULL	0	NULL	quality of dying	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of the literature revealed that the quality of dying and death construct is multidimensional , with 7 broad domains : physical experience , psychological experience , social experience , spiritual or existential experience , the nature of health care , life closure and death preparation , and the circumstances of death .
	manualset3
134922	4	406434	13	NULL	NULL	0	NULL	death construct	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of the literature revealed that the quality of dying and death construct is multidimensional , with 7 broad domains : physical experience , psychological experience , social experience , spiritual or existential experience , the nature of health care , life closure and death preparation , and the circumstances of death .
	manualset3
134923	5	406434	13	NULL	NULL	0	NULL	7 broad domains	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of the literature revealed that the quality of dying and death construct is multidimensional , with 7 broad domains : physical experience , psychological experience , social experience , spiritual or existential experience , the nature of health care , life closure and death preparation , and the circumstances of death .
	manualset3
134924	6	406434	13	NULL	NULL	0	NULL	physical experience	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of the literature revealed that the quality of dying and death construct is multidimensional , with 7 broad domains : physical experience , psychological experience , social experience , spiritual or existential experience , the nature of health care , life closure and death preparation , and the circumstances of death .
	manualset3
134925	7	406434	13	NULL	NULL	NULL	NULL	psychological experience	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Review of the literature revealed that the quality of dying and death construct is multidimensional , with 7 broad domains : physical experience , psychological experience , social experience , spiritual or existential experience , the nature of health care , life closure and death preparation , and the circumstances of death .
	manualset3
134926	8	406434	13	NULL	NULL	NULL	NULL	social experience	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Review of the literature revealed that the quality of dying and death construct is multidimensional , with 7 broad domains : physical experience , psychological experience , social experience , spiritual or existential experience , the nature of health care , life closure and death preparation , and the circumstances of death .
	manualset3
134927	9	406434	13	NULL	NULL	NULL	NULL	spiritual experience	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Review of the literature revealed that the quality of dying and death construct is multidimensional , with 7 broad domains : physical experience , psychological experience , social experience , spiritual or existential experience , the nature of health care , life closure and death preparation , and the circumstances of death .
	manualset3
134928	10	406434	13	NULL	NULL	NULL	NULL	existential experience	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Review of the literature revealed that the quality of dying and death construct is multidimensional , with 7 broad domains : physical experience , psychological experience , social experience , spiritual or existential experience , the nature of health care , life closure and death preparation , and the circumstances of death .
	manualset3
134929	11	406434	13	NULL	NULL	0	NULL	nature of health care 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of the literature revealed that the quality of dying and death construct is multidimensional , with 7 broad domains : physical experience , psychological experience , social experience , spiritual or existential experience , the nature of health care , life closure and death preparation , and the circumstances of death .
	manualset3
134930	12	406434	13	NULL	NULL	0	NULL	life closure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of the literature revealed that the quality of dying and death construct is multidimensional , with 7 broad domains : physical experience , psychological experience , social experience , spiritual or existential experience , the nature of health care , life closure and death preparation , and the circumstances of death .
	manualset3
134931	13	406434	13	NULL	NULL	0	NULL	 death preparation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of the literature revealed that the quality of dying and death construct is multidimensional , with 7 broad domains : physical experience , psychological experience , social experience , spiritual or existential experience , the nature of health care , life closure and death preparation , and the circumstances of death .
	manualset3
134932	14	406434	13	NULL	NULL	0	NULL	circumstances of death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of the literature revealed that the quality of dying and death construct is multidimensional , with 7 broad domains : physical experience , psychological experience , social experience , spiritual or existential experience , the nature of health care , life closure and death preparation , and the circumstances of death .
	manualset3
134933	1	406435	13	NULL	NULL	0	NULL	Review	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of trace elements in blood , serum and urine of the Belgian population and critical evaluation of their possible use as reference values .
	manualset3
134934	2	406435	13	NULL	NULL	0	NULL	trace elements in blood	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of trace elements in blood , serum and urine of the Belgian population and critical evaluation of their possible use as reference values .
	manualset3
134935	3	406435	13	NULL	NULL	0	NULL	serum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of trace elements in blood , serum and urine of the Belgian population and critical evaluation of their possible use as reference values .
	manualset3
134936	4	406435	13	NULL	NULL	0	NULL	urine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of trace elements in blood , serum and urine of the Belgian population and critical evaluation of their possible use as reference values .
	manualset3
134937	5	406435	13	NULL	NULL	0	NULL	Belgian population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of trace elements in blood , serum and urine of the Belgian population and critical evaluation of their possible use as reference values .
	manualset3
134938	6	406435	13	NULL	NULL	0	NULL	critical evaluation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of trace elements in blood , serum and urine of the Belgian population and critical evaluation of their possible use as reference values .
	manualset3
134939	7	406435	13	NULL	NULL	0	NULL	reference values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of trace elements in blood , serum and urine of the Belgian population and critical evaluation of their possible use as reference values .
	manualset3
134940	1	406436	13	NULL	NULL	NULL	NULL	Review 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Review of estimates of the global burden of injury and illness due to occupational exposures .
	manualset3
134941	2	406436	13	NULL	NULL	0	NULL	estimates	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of estimates of the global burden of injury and illness due to occupational exposures .
	manualset3
134942	3	406436	13	NULL	NULL	0	NULL	global burden of injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of estimates of the global burden of injury and illness due to occupational exposures .
	manualset3
134943	4	406436	13	NULL	NULL	0	NULL	 global burden of illness 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of estimates of the global burden of injury and illness due to occupational exposures .
	manualset3
134944	5	406436	13	NULL	NULL	0	NULL	occupational exposures 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Review of estimates of the global burden of injury and illness due to occupational exposures .
	manualset3
134950	1	406437	13	NULL	NULL	0	NULL	cyclic antidepressant cardiotoxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reviewing cyclic antidepressant cardiotoxicity : wheat and chaff .
	manualset3
134951	2	406437	13	NULL	NULL	NULL	NULL	wheat 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Reviewing cyclic antidepressant cardiotoxicity : wheat and chaff .
	manualset3
134952	3	406437	13	NULL	NULL	0	NULL	chaff	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Reviewing cyclic antidepressant cardiotoxicity : wheat and chaff .
	manualset3
134953	1	406438	13	NULL	NULL	0	NULL	Revision	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Revision of phylogenetic relationships in the antilopinae subfamily on the basis of the mitochondrial rRNA and beta-spectrin nuclear gene sequences .
	manualset3
134954	2	406438	13	NULL	NULL	0	NULL	phylogenetic relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Revision of phylogenetic relationships in the antilopinae subfamily on the basis of the mitochondrial rRNA and beta-spectrin nuclear gene sequences .
	manualset3
134955	3	406438	13	NULL	NULL	0	NULL	antilopinae subfamily	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Revision of phylogenetic relationships in the antilopinae subfamily on the basis of the mitochondrial rRNA and beta-spectrin nuclear gene sequences .
	manualset3
134956	4	406438	13	NULL	NULL	0	NULL	basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Revision of phylogenetic relationships in the antilopinae subfamily on the basis of the mitochondrial rRNA and beta-spectrin nuclear gene sequences .
	manualset3
134957	5	406438	13	NULL	NULL	0	NULL	mitochondrial rRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Revision of phylogenetic relationships in the antilopinae subfamily on the basis of the mitochondrial rRNA and beta-spectrin nuclear gene sequences .
	manualset3
134958	6	406438	13	NULL	NULL	0	NULL	beta-spectrin nuclear gene sequences 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Revision of phylogenetic relationships in the antilopinae subfamily on the basis of the mitochondrial rRNA and beta-spectrin nuclear gene sequences .
	manualset3
134959	1	406439	13	NULL	NULL	NULL	NULL	new ` Linc '	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A new ` Linc ' between noncoding RNAs and blood development .
	manualset3
134960	2	406439	13	NULL	NULL	0	NULL	noncoding RNAs 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A new ` Linc ' between noncoding RNAs and blood development .
	manualset3
134961	3	406439	13	NULL	NULL	0	NULL	blood development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A new ` Linc ' between noncoding RNAs and blood development .
	manualset3
134962	1	406440	13	NULL	NULL	0	NULL	Revisions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Revisions of the sticky network model that might address these issues are considered , as are alternatives including a model of cell wall biophysics in which cell wall polymers act as ` scaffolds ' to regulate the space available for microfibril movement .
	manualset3
134963	2	406440	13	NULL	NULL	0	NULL	network model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Revisions of the sticky network model that might address these issues are considered , as are alternatives including a model of cell wall biophysics in which cell wall polymers act as ` scaffolds ' to regulate the space available for microfibril movement .
	manualset3
134964	3	406440	13	NULL	NULL	0	NULL	issues	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Revisions of the sticky network model that might address these issues are considered , as are alternatives including a model of cell wall biophysics in which cell wall polymers act as ` scaffolds ' to regulate the space available for microfibril movement .
	manualset3
134965	4	406440	13	NULL	NULL	0	NULL	alternatives	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Revisions of the sticky network model that might address these issues are considered , as are alternatives including a model of cell wall biophysics in which cell wall polymers act as ` scaffolds ' to regulate the space available for microfibril movement .
	manualset3
134966	5	406440	13	NULL	NULL	0	NULL	 model of cell wall biophysics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Revisions of the sticky network model that might address these issues are considered , as are alternatives including a model of cell wall biophysics in which cell wall polymers act as ` scaffolds ' to regulate the space available for microfibril movement .
	manualset3
134967	6	406440	13	NULL	NULL	0	NULL	cell wall polymers	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Revisions of the sticky network model that might address these issues are considered , as are alternatives including a model of cell wall biophysics in which cell wall polymers act as ` scaffolds ' to regulate the space available for microfibril movement .
	manualset3
134968	7	406440	13	NULL	NULL	0	NULL	 ` scaffolds '	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Revisions of the sticky network model that might address these issues are considered , as are alternatives including a model of cell wall biophysics in which cell wall polymers act as ` scaffolds ' to regulate the space available for microfibril movement .
	manualset3
134969	8	406440	13	NULL	NULL	0	NULL	space 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Revisions of the sticky network model that might address these issues are considered , as are alternatives including a model of cell wall biophysics in which cell wall polymers act as ` scaffolds ' to regulate the space available for microfibril movement .
	manualset3
134970	9	406440	13	NULL	NULL	0	NULL	microfibril movement 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Revisions of the sticky network model that might address these issues are considered , as are alternatives including a model of cell wall biophysics in which cell wall polymers act as ` scaffolds ' to regulate the space available for microfibril movement .
	manualset3
134971	1	406441	13	NULL	NULL	0	NULL	RgpA-Kgp peptide-based immunogens	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	RgpA-Kgp peptide-based immunogens provide protection against Porphyromonas gingivalis challenge in a murine lesion model .
	manualset3
134972	2	406441	13	NULL	NULL	0	NULL	protection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	RgpA-Kgp peptide-based immunogens provide protection against Porphyromonas gingivalis challenge in a murine lesion model .
	manualset3
134973	3	406441	13	NULL	NULL	0	NULL	Porphyromonas gingivalis challenge 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	RgpA-Kgp peptide-based immunogens provide protection against Porphyromonas gingivalis challenge in a murine lesion model .
	manualset3
134974	4	406441	13	NULL	NULL	0	NULL	murine lesion model	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	RgpA-Kgp peptide-based immunogens provide protection against Porphyromonas gingivalis challenge in a murine lesion model .
	manualset3
134975	1	406442	13	NULL	NULL	0	NULL	Rhea	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Rhea includes enzyme-catalyzed reactions ( covering the IUBMB Enzyme Nomenclature list ) , transport reactions and spontaneously occurring reactions .
	manualset3
134976	2	406442	13	NULL	NULL	0	NULL	enzyme-catalyzed reactions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rhea includes enzyme-catalyzed reactions ( covering the IUBMB Enzyme Nomenclature list ) , transport reactions and spontaneously occurring reactions .
	manualset3
134977	3	406442	13	NULL	NULL	0	NULL	IUBMB Enzyme Nomenclature list 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Rhea includes enzyme-catalyzed reactions ( covering the IUBMB Enzyme Nomenclature list ) , transport reactions and spontaneously occurring reactions .
	manualset3
134978	4	406442	13	NULL	NULL	0	NULL	transport reactions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rhea includes enzyme-catalyzed reactions ( covering the IUBMB Enzyme Nomenclature list ) , transport reactions and spontaneously occurring reactions .
	manualset3
134979	5	406442	13	NULL	NULL	0	NULL	reactions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rhea includes enzyme-catalyzed reactions ( covering the IUBMB Enzyme Nomenclature list ) , transport reactions and spontaneously occurring reactions .
	manualset3
134980	1	406443	13	NULL	NULL	0	NULL	Rheb-CSVL 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Rheb-CSVL , a FTIs-resistant mutant , reduces the effects of FTIs on NSCLC cells .
	manualset3
134981	2	406443	13	NULL	NULL	0	NULL	FTIs-resistant mutant	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Rheb-CSVL , a FTIs-resistant mutant , reduces the effects of FTIs on NSCLC cells .
	manualset3
134982	3	406443	13	NULL	NULL	0	NULL	effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rheb-CSVL , a FTIs-resistant mutant , reduces the effects of FTIs on NSCLC cells .
	manualset3
134983	4	406443	13	NULL	NULL	0	NULL	FTIs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rheb-CSVL , a FTIs-resistant mutant , reduces the effects of FTIs on NSCLC cells .
	manualset3
134984	5	406443	13	NULL	NULL	0	NULL	NSCLC cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Rheb-CSVL , a FTIs-resistant mutant , reduces the effects of FTIs on NSCLC cells .
	manualset3
134985	1	406444	13	NULL	NULL	0	NULL	Rheological findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rheological findings in essential hypertension are increases in hematocrit , plasma fibrinogen , plasma and whole blood viscosity , and erythrocyte aggregability as well as impaired erythrocyte deformability .
	manualset3
134986	2	406444	13	NULL	NULL	0	NULL	hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rheological findings in essential hypertension are increases in hematocrit , plasma fibrinogen , plasma and whole blood viscosity , and erythrocyte aggregability as well as impaired erythrocyte deformability .
	manualset3
134987	3	406444	13	NULL	NULL	0	NULL	increases	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rheological findings in essential hypertension are increases in hematocrit , plasma fibrinogen , plasma and whole blood viscosity , and erythrocyte aggregability as well as impaired erythrocyte deformability .
	manualset3
134988	4	406444	13	NULL	NULL	0	NULL	hematocrit 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rheological findings in essential hypertension are increases in hematocrit , plasma fibrinogen , plasma and whole blood viscosity , and erythrocyte aggregability as well as impaired erythrocyte deformability .
	manualset3
134989	5	406444	13	NULL	NULL	0	NULL	plasma fibrinogen	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rheological findings in essential hypertension are increases in hematocrit , plasma fibrinogen , plasma and whole blood viscosity , and erythrocyte aggregability as well as impaired erythrocyte deformability .
	manualset3
134990	6	406444	13	NULL	NULL	0	NULL	 plasma viscosity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rheological findings in essential hypertension are increases in hematocrit , plasma fibrinogen , plasma and whole blood viscosity , and erythrocyte aggregability as well as impaired erythrocyte deformability .
	manualset3
134991	7	406444	13	NULL	NULL	0	NULL	whole blood viscosity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rheological findings in essential hypertension are increases in hematocrit , plasma fibrinogen , plasma and whole blood viscosity , and erythrocyte aggregability as well as impaired erythrocyte deformability .
	manualset3
134992	8	406444	13	NULL	NULL	0	NULL	erythrocyte aggregability 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rheological findings in essential hypertension are increases in hematocrit , plasma fibrinogen , plasma and whole blood viscosity , and erythrocyte aggregability as well as impaired erythrocyte deformability .
	manualset3
134993	9	406444	13	NULL	NULL	0	NULL	erythrocyte deformability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rheological findings in essential hypertension are increases in hematocrit , plasma fibrinogen , plasma and whole blood viscosity , and erythrocyte aggregability as well as impaired erythrocyte deformability .
	manualset3
134994	1	406445	13	NULL	NULL	0	NULL	Rhesus monkeys	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rhesus monkeys discriminated among eight possible directions of motion while directional signals were manipulated in visual area MT. One directional signal was generated by a visual stimulus and a second signal was introduced by electrically stimulating neurons that encoded a specific direction of motion .
	manualset3
134995	2	406445	13	NULL	NULL	0	NULL	eight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Rhesus monkeys discriminated among eight possible directions of motion while directional signals were manipulated in visual area MT. One directional signal was generated by a visual stimulus and a second signal was introduced by electrically stimulating neurons that encoded a specific direction of motion .
	manualset3
134996	3	406445	13	NULL	NULL	0	NULL	directions of motion	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rhesus monkeys discriminated among eight possible directions of motion while directional signals were manipulated in visual area MT. One directional signal was generated by a visual stimulus and a second signal was introduced by electrically stimulating neurons that encoded a specific direction of motion .
	manualset3
134997	4	406445	13	NULL	NULL	NULL	NULL	directional signals	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Rhesus monkeys discriminated among eight possible directions of motion while directional signals were manipulated in visual area MT. One directional signal was generated by a visual stimulus and a second signal was introduced by electrically stimulating neurons that encoded a specific direction of motion .
	manualset3
134998	5	406445	13	NULL	NULL	NULL	NULL	visual area MT	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Rhesus monkeys discriminated among eight possible directions of motion while directional signals were manipulated in visual area MT. One directional signal was generated by a visual stimulus and a second signal was introduced by electrically stimulating neurons that encoded a specific direction of motion .
	manualset3
134999	6	406445	13	NULL	NULL	0	NULL	One directional signal 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rhesus monkeys discriminated among eight possible directions of motion while directional signals were manipulated in visual area MT. One directional signal was generated by a visual stimulus and a second signal was introduced by electrically stimulating neurons that encoded a specific direction of motion .
	manualset3
135000	7	406445	13	NULL	NULL	0	NULL	visual stimulus	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rhesus monkeys discriminated among eight possible directions of motion while directional signals were manipulated in visual area MT. One directional signal was generated by a visual stimulus and a second signal was introduced by electrically stimulating neurons that encoded a specific direction of motion .
	manualset3
135001	8	406445	13	NULL	NULL	0	NULL	second signal	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rhesus monkeys discriminated among eight possible directions of motion while directional signals were manipulated in visual area MT. One directional signal was generated by a visual stimulus and a second signal was introduced by electrically stimulating neurons that encoded a specific direction of motion .
	manualset3
135002	9	406445	13	NULL	NULL	0	NULL	neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Rhesus monkeys discriminated among eight possible directions of motion while directional signals were manipulated in visual area MT. One directional signal was generated by a visual stimulus and a second signal was introduced by electrically stimulating neurons that encoded a specific direction of motion .
	manualset3
135003	10	406445	13	NULL	NULL	0	NULL	direction of motion	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rhesus monkeys discriminated among eight possible directions of motion while directional signals were manipulated in visual area MT. One directional signal was generated by a visual stimulus and a second signal was introduced by electrically stimulating neurons that encoded a specific direction of motion .
	manualset3
135004	1	406446	13	NULL	NULL	0	NULL	Rho GTPases 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Rho GTPases , which are key signaling enzymes in eukaryotes , are involved in sustaining the activation of sea urchin eggs ; however , their downstream effectors have not yet been characterized .
	manualset3
135005	2	406446	13	NULL	NULL	0	NULL	key signaling enzymes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Rho GTPases , which are key signaling enzymes in eukaryotes , are involved in sustaining the activation of sea urchin eggs ; however , their downstream effectors have not yet been characterized .
	manualset3
135006	3	406446	13	NULL	NULL	0	NULL	eukaryotes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rho GTPases , which are key signaling enzymes in eukaryotes , are involved in sustaining the activation of sea urchin eggs ; however , their downstream effectors have not yet been characterized .
	manualset3
135007	4	406446	13	NULL	NULL	0	NULL	activation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rho GTPases , which are key signaling enzymes in eukaryotes , are involved in sustaining the activation of sea urchin eggs ; however , their downstream effectors have not yet been characterized .
	manualset3
135008	5	406446	13	NULL	NULL	0	NULL	sea urchin eggs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Rho GTPases , which are key signaling enzymes in eukaryotes , are involved in sustaining the activation of sea urchin eggs ; however , their downstream effectors have not yet been characterized .
	manualset3
135009	6	406446	13	NULL	NULL	0	NULL	downstream effectors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Rho GTPases , which are key signaling enzymes in eukaryotes , are involved in sustaining the activation of sea urchin eggs ; however , their downstream effectors have not yet been characterized .
	manualset3
135010	1	406447	13	NULL	NULL	0	NULL	Rho family GTPases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Rho family GTPases appear to play an important role in the regulation of the actin cytoskeleton , but the mechanism of regulation is unknown .
	manualset3
135011	2	406447	13	NULL	NULL	0	NULL	role 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rho family GTPases appear to play an important role in the regulation of the actin cytoskeleton , but the mechanism of regulation is unknown .
	manualset3
135012	3	406447	13	NULL	NULL	0	NULL	regulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rho family GTPases appear to play an important role in the regulation of the actin cytoskeleton , but the mechanism of regulation is unknown .
	manualset3
135013	4	406447	13	NULL	NULL	0	NULL	actin cytoskeleton 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Rho family GTPases appear to play an important role in the regulation of the actin cytoskeleton , but the mechanism of regulation is unknown .
	manualset3
135014	5	406447	13	NULL	NULL	0	NULL	mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rho family GTPases appear to play an important role in the regulation of the actin cytoskeleton , but the mechanism of regulation is unknown .
	manualset3
135015	6	406447	13	NULL	NULL	0	NULL	regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rho family GTPases appear to play an important role in the regulation of the actin cytoskeleton , but the mechanism of regulation is unknown .
	manualset3
135016	1	406448	13	NULL	NULL	0	NULL	Rhyolite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rhyolite is the most viscous of liquid magmas , so it was surprising that on 2May 2008 at Chaitn Volcano , located in Chile 's southern Andean volcanic zone , rhyolitic magma migrated from more than 5km depth in less than 4hours ( ref .1 ) and erupted explosively with only two days of detected precursory seismic activity .
	manualset3
135018	2	406448	13	NULL	NULL	0	NULL	liquid magmas	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rhyolite is the most viscous of liquid magmas , so it was surprising that on 2May 2008 at Chaitn Volcano , located in Chile 's southern Andean volcanic zone , rhyolitic magma migrated from more than 5km depth in less than 4hours ( ref .1 ) and erupted explosively with only two days of detected precursory seismic activity .
	manualset3
135019	3	406448	13	NULL	NULL	0	NULL	2May 2008 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Rhyolite is the most viscous of liquid magmas , so it was surprising that on 2May 2008 at Chaitn Volcano , located in Chile 's southern Andean volcanic zone , rhyolitic magma migrated from more than 5km depth in less than 4hours ( ref .1 ) and erupted explosively with only two days of detected precursory seismic activity .
	manualset3
135020	4	406448	13	NULL	NULL	0	NULL	Chaitn Volcano	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Rhyolite is the most viscous of liquid magmas , so it was surprising that on 2May 2008 at Chaitn Volcano , located in Chile 's southern Andean volcanic zone , rhyolitic magma migrated from more than 5km depth in less than 4hours ( ref .1 ) and erupted explosively with only two days of detected precursory seismic activity .
	manualset3
135021	5	406448	13	NULL	NULL	0	NULL	Chile 's southern Andean volcanic zone	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Rhyolite is the most viscous of liquid magmas , so it was surprising that on 2May 2008 at Chaitn Volcano , located in Chile 's southern Andean volcanic zone , rhyolitic magma migrated from more than 5km depth in less than 4hours ( ref .1 ) and erupted explosively with only two days of detected precursory seismic activity .
	manualset3
135022	6	406448	13	NULL	NULL	0	NULL	rhyolitic magma	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rhyolite is the most viscous of liquid magmas , so it was surprising that on 2May 2008 at Chaitn Volcano , located in Chile 's southern Andean volcanic zone , rhyolitic magma migrated from more than 5km depth in less than 4hours ( ref .1 ) and erupted explosively with only two days of detected precursory seismic activity .
	manualset3
135023	7	406448	13	NULL	NULL	0	NULL	5km depth	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rhyolite is the most viscous of liquid magmas , so it was surprising that on 2May 2008 at Chaitn Volcano , located in Chile 's southern Andean volcanic zone , rhyolitic magma migrated from more than 5km depth in less than 4hours ( ref .1 ) and erupted explosively with only two days of detected precursory seismic activity .
	manualset3
135024	8	406448	13	NULL	NULL	0	NULL	4hours	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Rhyolite is the most viscous of liquid magmas , so it was surprising that on 2May 2008 at Chaitn Volcano , located in Chile 's southern Andean volcanic zone , rhyolitic magma migrated from more than 5km depth in less than 4hours ( ref .1 ) and erupted explosively with only two days of detected precursory seismic activity .
	manualset3
135025	9	406448	13	NULL	NULL	0	NULL	two days 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Rhyolite is the most viscous of liquid magmas , so it was surprising that on 2May 2008 at Chaitn Volcano , located in Chile 's southern Andean volcanic zone , rhyolitic magma migrated from more than 5km depth in less than 4hours ( ref .1 ) and erupted explosively with only two days of detected precursory seismic activity .
	manualset3
135026	10	406448	13	NULL	NULL	0	NULL	precursory seismic activity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rhyolite is the most viscous of liquid magmas , so it was surprising that on 2May 2008 at Chaitn Volcano , located in Chile 's southern Andean volcanic zone , rhyolitic magma migrated from more than 5km depth in less than 4hours ( ref .1 ) and erupted explosively with only two days of detected precursory seismic activity .
	manualset3
135027	1	406449	13	NULL	NULL	0	NULL	Rhyolite magma	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rhyolite magma has fuelled some of the Earth 's largest explosive volcanic eruptions .
	manualset3
135028	2	406449	13	NULL	NULL	0	NULL	Earth 's	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Rhyolite magma has fuelled some of the Earth 's largest explosive volcanic eruptions .
	manualset3
135029	3	406449	13	NULL	NULL	0	NULL	explosive volcanic eruptions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rhyolite magma has fuelled some of the Earth 's largest explosive volcanic eruptions .
	manualset3
135030	1	406450	13	NULL	NULL	0	NULL	Ribonucleoside triphosphates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ribonucleoside triphosphates are not required , although they stimulate DNA synthesis .
	manualset3
135031	2	406450	13	NULL	NULL	0	NULL	DNA synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ribonucleoside triphosphates are not required , although they stimulate DNA synthesis .
	manualset3
135032	1	406451	13	NULL	NULL	0	NULL	Rice transitory yellowing virus ( RTYV ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rice transitory yellowing virus ( RTYV ) , a member of the genus Nucleorhabdovirus , is closely related to or synonymous with rice yellow stunt virus ( RYSV ) .
	manualset3
135033	2	406451	13	NULL	NULL	0	NULL	member 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rice transitory yellowing virus ( RTYV ) , a member of the genus Nucleorhabdovirus , is closely related to or synonymous with rice yellow stunt virus ( RYSV ) .
	manualset3
135034	3	406451	13	NULL	NULL	0	NULL	genus Nucleorhabdovirus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rice transitory yellowing virus ( RTYV ) , a member of the genus Nucleorhabdovirus , is closely related to or synonymous with rice yellow stunt virus ( RYSV ) .
	manualset3
135035	4	406451	13	NULL	NULL	0	NULL	rice yellow stunt virus ( RYSV ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rice transitory yellowing virus ( RTYV ) , a member of the genus Nucleorhabdovirus , is closely related to or synonymous with rice yellow stunt virus ( RYSV ) .
	manualset3
135036	1	406452	13	NULL	NULL	0	NULL	normal controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Right-hemisphere-damaged and normal controls showed no performance deficit for judgments of monotone sentences .
	manualset3
135037	2	406452	13	NULL	NULL	0	NULL	performance deficit	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Right-hemisphere-damaged and normal controls showed no performance deficit for judgments of monotone sentences .
	manualset3
135038	3	406452	13	NULL	NULL	0	NULL	judgments	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Right-hemisphere-damaged and normal controls showed no performance deficit for judgments of monotone sentences .
	manualset3
135039	4	406452	13	NULL	NULL	0	NULL	monotone sentences 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Right-hemisphere-damaged and normal controls showed no performance deficit for judgments of monotone sentences .
	manualset3
135040	1	406453	13	NULL	NULL	0	NULL	Right bundle branch block	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Right bundle branch block was present in 21 ( 70 % ) , documented supraventricular tachycardia in seven ( 23 % ) , and Wolff-Parkinson-White syndrome in three ( 10 % ) .
	manualset3
135041	2	406453	13	NULL	NULL	0	NULL	21 ( 70 % ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Right bundle branch block was present in 21 ( 70 % ) , documented supraventricular tachycardia in seven ( 23 % ) , and Wolff-Parkinson-White syndrome in three ( 10 % ) .
	manualset3
135042	3	406453	13	NULL	NULL	0	NULL	supraventricular tachycardia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Right bundle branch block was present in 21 ( 70 % ) , documented supraventricular tachycardia in seven ( 23 % ) , and Wolff-Parkinson-White syndrome in three ( 10 % ) .
	manualset3
135043	4	406453	13	NULL	NULL	0	NULL	seven ( 23 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Right bundle branch block was present in 21 ( 70 % ) , documented supraventricular tachycardia in seven ( 23 % ) , and Wolff-Parkinson-White syndrome in three ( 10 % ) .
	manualset3
135044	5	406453	13	NULL	NULL	0	NULL	Wolff-Parkinson-White syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Right bundle branch block was present in 21 ( 70 % ) , documented supraventricular tachycardia in seven ( 23 % ) , and Wolff-Parkinson-White syndrome in three ( 10 % ) .
	manualset3
135045	6	406453	13	NULL	NULL	0	NULL	three ( 10 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Right bundle branch block was present in 21 ( 70 % ) , documented supraventricular tachycardia in seven ( 23 % ) , and Wolff-Parkinson-White syndrome in three ( 10 % ) .
	manualset3
135046	1	406454	13	NULL	NULL	0	NULL	Rigorous testing 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Rigorous testing of kava raw material is urgently advised , in addition to Pan-Pacific kava manufacturing quality standards .
	manualset3
135047	2	406454	13	NULL	NULL	0	NULL	kava raw material 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Rigorous testing of kava raw material is urgently advised , in addition to Pan-Pacific kava manufacturing quality standards .
	manualset3
135048	3	406454	13	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rigorous testing of kava raw material is urgently advised , in addition to Pan-Pacific kava manufacturing quality standards .
	manualset3
135049	4	406454	13	NULL	NULL	0	NULL	Pan-Pacific kava	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rigorous testing of kava raw material is urgently advised , in addition to Pan-Pacific kava manufacturing quality standards .
	manualset3
135050	5	406454	13	NULL	NULL	0	NULL	quality standards 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rigorous testing of kava raw material is urgently advised , in addition to Pan-Pacific kava manufacturing quality standards .
	manualset3
135051	1	406455	13	NULL	NULL	0	NULL	weekend effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rigorously investigating the ` weekend effect ' on short-term mortality for patients admitted with stroke .
	manualset3
135052	2	406455	13	NULL	NULL	0	NULL	short-term mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rigorously investigating the ` weekend effect ' on short-term mortality for patients admitted with stroke .
	manualset3
135053	3	406455	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Rigorously investigating the ` weekend effect ' on short-term mortality for patients admitted with stroke .
	manualset3
135054	4	406455	13	NULL	NULL	0	NULL	stroke	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rigorously investigating the ` weekend effect ' on short-term mortality for patients admitted with stroke .
	manualset3
135055	1	406456	13	NULL	NULL	0	NULL	Riluzole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Riluzole treatment also reversed CUS-induced reductions in glial metabolism and GFAP mRNA expression .
	manualset3
135056	2	406456	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Riluzole treatment also reversed CUS-induced reductions in glial metabolism and GFAP mRNA expression .
	manualset3
135057	3	406456	13	NULL	NULL	0	NULL	CUS-induced reductions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Riluzole treatment also reversed CUS-induced reductions in glial metabolism and GFAP mRNA expression .
	manualset3
135058	4	406456	13	NULL	NULL	0	NULL	glial metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Riluzole treatment also reversed CUS-induced reductions in glial metabolism and GFAP mRNA expression .
	manualset3
135059	5	406456	13	NULL	NULL	0	NULL	GFAP mRNA expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Riluzole treatment also reversed CUS-induced reductions in glial metabolism and GFAP mRNA expression .
	manualset3
135060	1	406457	13	NULL	NULL	0	NULL	Ring-14	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Ring-14 and trisomy 14q in the same child .
	manualset3
135061	2	406457	13	NULL	NULL	0	NULL	trisomy 14q	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Ring-14 and trisomy 14q in the same child .
	manualset3
135062	3	406457	13	NULL	NULL	0	NULL	child	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Ring-14 and trisomy 14q in the same child .
	manualset3
135063	1	406458	13	NULL	NULL	0	NULL	Ring preparations 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ring preparations of small intramyometrial and intracervical arteries were dissected and mounted in organ baths ; isometric tension was recorded and responses to contractile agents were studied .
	manualset3
135064	2	406458	13	NULL	NULL	0	NULL	small intramyometrial arteries 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ring preparations of small intramyometrial and intracervical arteries were dissected and mounted in organ baths ; isometric tension was recorded and responses to contractile agents were studied .
	manualset3
135065	3	406458	13	NULL	NULL	0	NULL	intracervical arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ring preparations of small intramyometrial and intracervical arteries were dissected and mounted in organ baths ; isometric tension was recorded and responses to contractile agents were studied .
	manualset3
135066	4	406458	13	NULL	NULL	0	NULL	organ baths	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Ring preparations of small intramyometrial and intracervical arteries were dissected and mounted in organ baths ; isometric tension was recorded and responses to contractile agents were studied .
	manualset3
135067	5	406458	13	NULL	NULL	0	NULL	isometric tension	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ring preparations of small intramyometrial and intracervical arteries were dissected and mounted in organ baths ; isometric tension was recorded and responses to contractile agents were studied .
	manualset3
135068	6	406458	13	NULL	NULL	0	NULL	responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ring preparations of small intramyometrial and intracervical arteries were dissected and mounted in organ baths ; isometric tension was recorded and responses to contractile agents were studied .
	manualset3
135069	7	406458	13	NULL	NULL	0	NULL	contractile agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ring preparations of small intramyometrial and intracervical arteries were dissected and mounted in organ baths ; isometric tension was recorded and responses to contractile agents were studied .
	manualset3
135070	1	406459	13	NULL	NULL	0	NULL	Risk assessment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk assessment due to ingestion of natural radionuclides and heavy metals in the milk samples : a case study from a proposed uranium mining area , Jharkhand .
	manualset3
135071	2	406459	13	NULL	NULL	0	NULL	ingestion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk assessment due to ingestion of natural radionuclides and heavy metals in the milk samples : a case study from a proposed uranium mining area , Jharkhand .
	manualset3
135072	3	406459	13	NULL	NULL	0	NULL	natural radionuclides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk assessment due to ingestion of natural radionuclides and heavy metals in the milk samples : a case study from a proposed uranium mining area , Jharkhand .
	manualset3
135073	4	406459	13	NULL	NULL	0	NULL	heavy metals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk assessment due to ingestion of natural radionuclides and heavy metals in the milk samples : a case study from a proposed uranium mining area , Jharkhand .
	manualset3
135074	5	406459	13	NULL	NULL	0	NULL	milk samples 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk assessment due to ingestion of natural radionuclides and heavy metals in the milk samples : a case study from a proposed uranium mining area , Jharkhand .
	manualset3
135075	6	406459	13	NULL	NULL	0	NULL	case study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk assessment due to ingestion of natural radionuclides and heavy metals in the milk samples : a case study from a proposed uranium mining area , Jharkhand .
	manualset3
135076	7	406459	13	NULL	NULL	0	NULL	uranium mining area	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk assessment due to ingestion of natural radionuclides and heavy metals in the milk samples : a case study from a proposed uranium mining area , Jharkhand .
	manualset3
135077	8	406459	13	NULL	NULL	0	NULL	Jharkhand 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk assessment due to ingestion of natural radionuclides and heavy metals in the milk samples : a case study from a proposed uranium mining area , Jharkhand .
	manualset3
135078	1	406460	13	NULL	NULL	0	NULL	Risk evaluation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk evaluation of UVB therapy for psoriasis : comparison of calculated risk for UVB therapy and observed risk in PUVA-treated patients .
	manualset3
135079	2	406460	13	NULL	NULL	0	NULL	UVB therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk evaluation of UVB therapy for psoriasis : comparison of calculated risk for UVB therapy and observed risk in PUVA-treated patients .
	manualset3
135080	3	406460	13	NULL	NULL	0	NULL	psoriasis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk evaluation of UVB therapy for psoriasis : comparison of calculated risk for UVB therapy and observed risk in PUVA-treated patients .
	manualset3
135081	4	406460	13	NULL	NULL	0	NULL	comparison 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk evaluation of UVB therapy for psoriasis : comparison of calculated risk for UVB therapy and observed risk in PUVA-treated patients .
	manualset3
135082	5	406460	13	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk evaluation of UVB therapy for psoriasis : comparison of calculated risk for UVB therapy and observed risk in PUVA-treated patients .
	manualset3
135083	6	406460	13	NULL	NULL	0	NULL	UVB therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk evaluation of UVB therapy for psoriasis : comparison of calculated risk for UVB therapy and observed risk in PUVA-treated patients .
	manualset3
135084	7	406460	13	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk evaluation of UVB therapy for psoriasis : comparison of calculated risk for UVB therapy and observed risk in PUVA-treated patients .
	manualset3
135085	8	406460	13	NULL	NULL	0	NULL	PUVA-treated patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk evaluation of UVB therapy for psoriasis : comparison of calculated risk for UVB therapy and observed risk in PUVA-treated patients .
	manualset3
135086	1	406461	13	NULL	NULL	0	NULL	new approach 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A new approach to combretastatin D2 .
	manualset3
135087	2	406461	13	NULL	NULL	0	NULL	combretastatin D2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A new approach to combretastatin D2 .
	manualset3
135088	1	406462	13	NULL	NULL	0	NULL	Risk factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk factors for testicular germ cell tumors by histological tumor type .
	manualset3
135089	2	406462	13	NULL	NULL	0	NULL	testicular germ cell tumors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk factors for testicular germ cell tumors by histological tumor type .
	manualset3
135090	3	406462	13	NULL	NULL	0	NULL	histological tumor type	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk factors for testicular germ cell tumors by histological tumor type .
	manualset3
135091	1	406463	13	NULL	NULL	0	NULL	Risk factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk factors for this outcome included a history of coronary artery disease , pulmonary edema seen on a chest x-ray , or a subsequent myocardial infarction .
	manualset3
135092	2	406463	13	NULL	NULL	0	NULL	outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk factors for this outcome included a history of coronary artery disease , pulmonary edema seen on a chest x-ray , or a subsequent myocardial infarction .
	manualset3
135093	3	406463	13	NULL	NULL	0	NULL	history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk factors for this outcome included a history of coronary artery disease , pulmonary edema seen on a chest x-ray , or a subsequent myocardial infarction .
	manualset3
135094	4	406463	13	NULL	NULL	0	NULL	coronary artery disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk factors for this outcome included a history of coronary artery disease , pulmonary edema seen on a chest x-ray , or a subsequent myocardial infarction .
	manualset3
135095	5	406463	13	NULL	NULL	0	NULL	pulmonary edema	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk factors for this outcome included a history of coronary artery disease , pulmonary edema seen on a chest x-ray , or a subsequent myocardial infarction .
	manualset3
135096	6	406463	13	NULL	NULL	0	NULL	chest x-ray	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk factors for this outcome included a history of coronary artery disease , pulmonary edema seen on a chest x-ray , or a subsequent myocardial infarction .
	manualset3
135097	7	406463	13	NULL	NULL	0	NULL	myocardial infarction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk factors for this outcome included a history of coronary artery disease , pulmonary edema seen on a chest x-ray , or a subsequent myocardial infarction .
	manualset3
135578	1	406464	13	NULL	NULL	0	NULL	Risk groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk groups , such as hemophiliacs ( 70-95 % ) , i.v. drug addicts ( 30-80 % ) and hemodialysis patients ( 0-45 % ) , show a high prevalence of chronic HCV infection .
	manualset3
135579	2	406464	13	NULL	NULL	0	NULL	hemophiliacs	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk groups , such as hemophiliacs ( 70-95 % ) , i.v. drug addicts ( 30-80 % ) and hemodialysis patients ( 0-45 % ) , show a high prevalence of chronic HCV infection .
	manualset3
135580	3	406464	13	NULL	NULL	0	NULL	70-95 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk groups , such as hemophiliacs ( 70-95 % ) , i.v. drug addicts ( 30-80 % ) and hemodialysis patients ( 0-45 % ) , show a high prevalence of chronic HCV infection .
	manualset3
135581	4	406464	13	NULL	NULL	0	NULL	drug addicts	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk groups , such as hemophiliacs ( 70-95 % ) , i.v. drug addicts ( 30-80 % ) and hemodialysis patients ( 0-45 % ) , show a high prevalence of chronic HCV infection .
	manualset3
135582	5	406464	13	NULL	NULL	0	NULL	30-80 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk groups , such as hemophiliacs ( 70-95 % ) , i.v. drug addicts ( 30-80 % ) and hemodialysis patients ( 0-45 % ) , show a high prevalence of chronic HCV infection .
	manualset3
135583	6	406464	13	NULL	NULL	0	NULL	hemodialysis patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk groups , such as hemophiliacs ( 70-95 % ) , i.v. drug addicts ( 30-80 % ) and hemodialysis patients ( 0-45 % ) , show a high prevalence of chronic HCV infection .
	manualset3
135584	7	406464	13	NULL	NULL	0	NULL	0-45 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk groups , such as hemophiliacs ( 70-95 % ) , i.v. drug addicts ( 30-80 % ) and hemodialysis patients ( 0-45 % ) , show a high prevalence of chronic HCV infection .
	manualset3
135585	8	406464	13	NULL	NULL	0	NULL	prevalence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk groups , such as hemophiliacs ( 70-95 % ) , i.v. drug addicts ( 30-80 % ) and hemodialysis patients ( 0-45 % ) , show a high prevalence of chronic HCV infection .
	manualset3
135586	9	406464	13	NULL	NULL	0	NULL	 chronic HCV infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk groups , such as hemophiliacs ( 70-95 % ) , i.v. drug addicts ( 30-80 % ) and hemodialysis patients ( 0-45 % ) , show a high prevalence of chronic HCV infection .
	manualset3
135587	1	406465	13	NULL	NULL	0	NULL	Risk of herpes zoster	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk of herpes zoster in children with leukemia : varicella vaccine compared with history of chickenpox .
	manualset3
135588	2	406465	13	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk of herpes zoster in children with leukemia : varicella vaccine compared with history of chickenpox .
	manualset3
135589	3	406465	13	NULL	NULL	0	NULL	leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk of herpes zoster in children with leukemia : varicella vaccine compared with history of chickenpox .
	manualset3
135590	4	406465	13	NULL	NULL	0	NULL	varicella vaccine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk of herpes zoster in children with leukemia : varicella vaccine compared with history of chickenpox .
	manualset3
135591	5	406465	13	NULL	NULL	0	NULL	history of chickenpox	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk of herpes zoster in children with leukemia : varicella vaccine compared with history of chickenpox .
	manualset3
135592	1	406466	13	NULL	NULL	0	NULL	Risks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Risks for DSM-III-R anxiety and affective disorders and `` subdisorder '' ( nonimpairing ) irrational social fears , among directly interviewed first-degree relatives ( n = 83 ) of probands who met criteria for social phobia but for no other lifetime anxiety disorder diagnosis , were contrasted to risks for disorder among similarly evaluated relatives ( n = 231 ) of never mentally ill controls .
	manualset3
135593	2	406466	13	NULL	NULL	0	NULL	DSM-III-R anxiety	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Risks for DSM-III-R anxiety and affective disorders and `` subdisorder '' ( nonimpairing ) irrational social fears , among directly interviewed first-degree relatives ( n = 83 ) of probands who met criteria for social phobia but for no other lifetime anxiety disorder diagnosis , were contrasted to risks for disorder among similarly evaluated relatives ( n = 231 ) of never mentally ill controls .
	manualset3
135594	3	406466	13	NULL	NULL	0	NULL	affective disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Risks for DSM-III-R anxiety and affective disorders and `` subdisorder '' ( nonimpairing ) irrational social fears , among directly interviewed first-degree relatives ( n = 83 ) of probands who met criteria for social phobia but for no other lifetime anxiety disorder diagnosis , were contrasted to risks for disorder among similarly evaluated relatives ( n = 231 ) of never mentally ill controls .
	manualset3
135595	4	406466	13	NULL	NULL	0	NULL	`` subdisorder '' ( nonimpairing ) irrational social fears	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Risks for DSM-III-R anxiety and affective disorders and `` subdisorder '' ( nonimpairing ) irrational social fears , among directly interviewed first-degree relatives ( n = 83 ) of probands who met criteria for social phobia but for no other lifetime anxiety disorder diagnosis , were contrasted to risks for disorder among similarly evaluated relatives ( n = 231 ) of never mentally ill controls .
	manualset3
135596	5	406466	13	NULL	NULL	0	NULL	 first-degree relatives	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Risks for DSM-III-R anxiety and affective disorders and `` subdisorder '' ( nonimpairing ) irrational social fears , among directly interviewed first-degree relatives ( n = 83 ) of probands who met criteria for social phobia but for no other lifetime anxiety disorder diagnosis , were contrasted to risks for disorder among similarly evaluated relatives ( n = 231 ) of never mentally ill controls .
	manualset3
135597	6	406466	13	NULL	NULL	0	NULL	n = 83	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Risks for DSM-III-R anxiety and affective disorders and `` subdisorder '' ( nonimpairing ) irrational social fears , among directly interviewed first-degree relatives ( n = 83 ) of probands who met criteria for social phobia but for no other lifetime anxiety disorder diagnosis , were contrasted to risks for disorder among similarly evaluated relatives ( n = 231 ) of never mentally ill controls .
	manualset3
135598	7	406466	13	NULL	NULL	0	NULL	probands 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Risks for DSM-III-R anxiety and affective disorders and `` subdisorder '' ( nonimpairing ) irrational social fears , among directly interviewed first-degree relatives ( n = 83 ) of probands who met criteria for social phobia but for no other lifetime anxiety disorder diagnosis , were contrasted to risks for disorder among similarly evaluated relatives ( n = 231 ) of never mentally ill controls .
	manualset3
135599	8	406466	13	NULL	NULL	0	NULL	criteria	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Risks for DSM-III-R anxiety and affective disorders and `` subdisorder '' ( nonimpairing ) irrational social fears , among directly interviewed first-degree relatives ( n = 83 ) of probands who met criteria for social phobia but for no other lifetime anxiety disorder diagnosis , were contrasted to risks for disorder among similarly evaluated relatives ( n = 231 ) of never mentally ill controls .
	manualset3
135600	9	406466	13	NULL	NULL	0	NULL	social phobia 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Risks for DSM-III-R anxiety and affective disorders and `` subdisorder '' ( nonimpairing ) irrational social fears , among directly interviewed first-degree relatives ( n = 83 ) of probands who met criteria for social phobia but for no other lifetime anxiety disorder diagnosis , were contrasted to risks for disorder among similarly evaluated relatives ( n = 231 ) of never mentally ill controls .
	manualset3
135601	10	406466	13	NULL	NULL	0	NULL	lifetime anxiety disorder diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Risks for DSM-III-R anxiety and affective disorders and `` subdisorder '' ( nonimpairing ) irrational social fears , among directly interviewed first-degree relatives ( n = 83 ) of probands who met criteria for social phobia but for no other lifetime anxiety disorder diagnosis , were contrasted to risks for disorder among similarly evaluated relatives ( n = 231 ) of never mentally ill controls .
	manualset3
135602	11	406466	13	NULL	NULL	0	NULL	risks 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Risks for DSM-III-R anxiety and affective disorders and `` subdisorder '' ( nonimpairing ) irrational social fears , among directly interviewed first-degree relatives ( n = 83 ) of probands who met criteria for social phobia but for no other lifetime anxiety disorder diagnosis , were contrasted to risks for disorder among similarly evaluated relatives ( n = 231 ) of never mentally ill controls .
	manualset3
135603	12	406466	13	NULL	NULL	0	NULL	disorder	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Risks for DSM-III-R anxiety and affective disorders and `` subdisorder '' ( nonimpairing ) irrational social fears , among directly interviewed first-degree relatives ( n = 83 ) of probands who met criteria for social phobia but for no other lifetime anxiety disorder diagnosis , were contrasted to risks for disorder among similarly evaluated relatives ( n = 231 ) of never mentally ill controls .
	manualset3
135604	13	406466	13	NULL	NULL	0	NULL	relatives	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Risks for DSM-III-R anxiety and affective disorders and `` subdisorder '' ( nonimpairing ) irrational social fears , among directly interviewed first-degree relatives ( n = 83 ) of probands who met criteria for social phobia but for no other lifetime anxiety disorder diagnosis , were contrasted to risks for disorder among similarly evaluated relatives ( n = 231 ) of never mentally ill controls .
	manualset3
135605	14	406466	13	NULL	NULL	0	NULL	n = 231	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Risks for DSM-III-R anxiety and affective disorders and `` subdisorder '' ( nonimpairing ) irrational social fears , among directly interviewed first-degree relatives ( n = 83 ) of probands who met criteria for social phobia but for no other lifetime anxiety disorder diagnosis , were contrasted to risks for disorder among similarly evaluated relatives ( n = 231 ) of never mentally ill controls .
	manualset3
135606	15	406466	13	NULL	NULL	0	NULL	mentally ill controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Risks for DSM-III-R anxiety and affective disorders and `` subdisorder '' ( nonimpairing ) irrational social fears , among directly interviewed first-degree relatives ( n = 83 ) of probands who met criteria for social phobia but for no other lifetime anxiety disorder diagnosis , were contrasted to risks for disorder among similarly evaluated relatives ( n = 231 ) of never mentally ill controls .
	manualset3
135607	1	406467	13	NULL	NULL	0	NULL	Risperidone 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Risperidone alone or in combination for acute mania .
	manualset3
135608	2	406467	13	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Risperidone alone or in combination for acute mania .
	manualset3
135609	3	406467	13	NULL	NULL	0	NULL	acute mania 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Risperidone alone or in combination for acute mania .
	manualset3
135610	1	406468	13	NULL	NULL	0	NULL	Ro 22-4839	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ro 22-4839 was found to dilate basilar and middle cerebral arteries and to non-selectively antagonize submaximal contraction of these arteries under the treatment of various constrictors ( K + , Ca2 + , PGF2 alpha ( dinoprost ) , serotonin and incubated blood ) with IC50 values ranging from 0.043 to 1.69 mumol/l .
	manualset3
135611	2	406468	13	NULL	NULL	0	NULL	basilar cerebral arteries 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ro 22-4839 was found to dilate basilar and middle cerebral arteries and to non-selectively antagonize submaximal contraction of these arteries under the treatment of various constrictors ( K + , Ca2 + , PGF2 alpha ( dinoprost ) , serotonin and incubated blood ) with IC50 values ranging from 0.043 to 1.69 mumol/l .
	manualset3
135612	3	406468	13	NULL	NULL	0	NULL	middle cerebral arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ro 22-4839 was found to dilate basilar and middle cerebral arteries and to non-selectively antagonize submaximal contraction of these arteries under the treatment of various constrictors ( K + , Ca2 + , PGF2 alpha ( dinoprost ) , serotonin and incubated blood ) with IC50 values ranging from 0.043 to 1.69 mumol/l .
	manualset3
135613	4	406468	13	NULL	NULL	0	NULL	submaximal contraction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ro 22-4839 was found to dilate basilar and middle cerebral arteries and to non-selectively antagonize submaximal contraction of these arteries under the treatment of various constrictors ( K + , Ca2 + , PGF2 alpha ( dinoprost ) , serotonin and incubated blood ) with IC50 values ranging from 0.043 to 1.69 mumol/l .
	manualset3
135614	5	406468	13	NULL	NULL	0	NULL	arteries 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ro 22-4839 was found to dilate basilar and middle cerebral arteries and to non-selectively antagonize submaximal contraction of these arteries under the treatment of various constrictors ( K + , Ca2 + , PGF2 alpha ( dinoprost ) , serotonin and incubated blood ) with IC50 values ranging from 0.043 to 1.69 mumol/l .
	manualset3
135615	6	406468	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ro 22-4839 was found to dilate basilar and middle cerebral arteries and to non-selectively antagonize submaximal contraction of these arteries under the treatment of various constrictors ( K + , Ca2 + , PGF2 alpha ( dinoprost ) , serotonin and incubated blood ) with IC50 values ranging from 0.043 to 1.69 mumol/l .
	manualset3
135616	7	406468	13	NULL	NULL	0	NULL	various constrictors 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ro 22-4839 was found to dilate basilar and middle cerebral arteries and to non-selectively antagonize submaximal contraction of these arteries under the treatment of various constrictors ( K + , Ca2 + , PGF2 alpha ( dinoprost ) , serotonin and incubated blood ) with IC50 values ranging from 0.043 to 1.69 mumol/l .
	manualset3
135617	8	406468	13	NULL	NULL	0	NULL	K +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Ro 22-4839 was found to dilate basilar and middle cerebral arteries and to non-selectively antagonize submaximal contraction of these arteries under the treatment of various constrictors ( K + , Ca2 + , PGF2 alpha ( dinoprost ) , serotonin and incubated blood ) with IC50 values ranging from 0.043 to 1.69 mumol/l .
	manualset3
135618	9	406468	13	NULL	NULL	0	NULL	Ca2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Ro 22-4839 was found to dilate basilar and middle cerebral arteries and to non-selectively antagonize submaximal contraction of these arteries under the treatment of various constrictors ( K + , Ca2 + , PGF2 alpha ( dinoprost ) , serotonin and incubated blood ) with IC50 values ranging from 0.043 to 1.69 mumol/l .
	manualset3
135619	10	406468	13	NULL	NULL	0	NULL	PGF2 alpha ( dinoprost )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Ro 22-4839 was found to dilate basilar and middle cerebral arteries and to non-selectively antagonize submaximal contraction of these arteries under the treatment of various constrictors ( K + , Ca2 + , PGF2 alpha ( dinoprost ) , serotonin and incubated blood ) with IC50 values ranging from 0.043 to 1.69 mumol/l .
	manualset3
135620	11	406468	13	NULL	NULL	0	NULL	serotonin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ro 22-4839 was found to dilate basilar and middle cerebral arteries and to non-selectively antagonize submaximal contraction of these arteries under the treatment of various constrictors ( K + , Ca2 + , PGF2 alpha ( dinoprost ) , serotonin and incubated blood ) with IC50 values ranging from 0.043 to 1.69 mumol/l .
	manualset3
135621	12	406468	13	NULL	NULL	0	NULL	blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Ro 22-4839 was found to dilate basilar and middle cerebral arteries and to non-selectively antagonize submaximal contraction of these arteries under the treatment of various constrictors ( K + , Ca2 + , PGF2 alpha ( dinoprost ) , serotonin and incubated blood ) with IC50 values ranging from 0.043 to 1.69 mumol/l .
	manualset3
135622	13	406468	13	NULL	NULL	0	NULL	IC50 values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ro 22-4839 was found to dilate basilar and middle cerebral arteries and to non-selectively antagonize submaximal contraction of these arteries under the treatment of various constrictors ( K + , Ca2 + , PGF2 alpha ( dinoprost ) , serotonin and incubated blood ) with IC50 values ranging from 0.043 to 1.69 mumol/l .
	manualset3
135623	14	406468	13	NULL	NULL	0	NULL	0.043 to 1.69 mumol/l 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ro 22-4839 was found to dilate basilar and middle cerebral arteries and to non-selectively antagonize submaximal contraction of these arteries under the treatment of various constrictors ( K + , Ca2 + , PGF2 alpha ( dinoprost ) , serotonin and incubated blood ) with IC50 values ranging from 0.043 to 1.69 mumol/l .
	manualset3
135624	1	406469	13	NULL	NULL	0	NULL	approach	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A new approach to define the upper normal limits of ambulatory blood pressure .
	manualset3
135625	2	406469	13	NULL	NULL	0	NULL	upper normal limits	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A new approach to define the upper normal limits of ambulatory blood pressure .
	manualset3
135626	3	406469	13	NULL	NULL	0	NULL	ambulatory blood pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A new approach to define the upper normal limits of ambulatory blood pressure .
	manualset3
135627	1	406470	13	NULL	NULL	0	NULL	Robotic-assisted laparoscopic surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Robotic-assisted laparoscopic surgery has been applied to pediatric surgery , especially for technically challenging reconstructive procedures owing to the improved suturing capabilities over pure laparoscopic techniques when using fine suture material .
	manualset3
135628	2	406470	13	NULL	NULL	0	NULL	pediatric surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Robotic-assisted laparoscopic surgery has been applied to pediatric surgery , especially for technically challenging reconstructive procedures owing to the improved suturing capabilities over pure laparoscopic techniques when using fine suture material .
	manualset3
135629	3	406470	13	NULL	NULL	0	NULL	reconstructive procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Robotic-assisted laparoscopic surgery has been applied to pediatric surgery , especially for technically challenging reconstructive procedures owing to the improved suturing capabilities over pure laparoscopic techniques when using fine suture material .
	manualset3
135630	4	406470	13	NULL	NULL	0	NULL	capabilities 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Robotic-assisted laparoscopic surgery has been applied to pediatric surgery , especially for technically challenging reconstructive procedures owing to the improved suturing capabilities over pure laparoscopic techniques when using fine suture material .
	manualset3
135631	5	406470	13	NULL	NULL	0	NULL	pure laparoscopic techniques 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Robotic-assisted laparoscopic surgery has been applied to pediatric surgery , especially for technically challenging reconstructive procedures owing to the improved suturing capabilities over pure laparoscopic techniques when using fine suture material .
	manualset3
135632	6	406470	13	NULL	NULL	0	NULL	fine suture material	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Robotic-assisted laparoscopic surgery has been applied to pediatric surgery , especially for technically challenging reconstructive procedures owing to the improved suturing capabilities over pure laparoscopic techniques when using fine suture material .
	manualset3
135633	1	406471	13	NULL	NULL	0	NULL	Robotic nerve-sparing radical parametrectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Robotic nerve-sparing radical parametrectomy : feasibility and technique .
	manualset3
135634	2	406471	13	NULL	NULL	0	NULL	feasibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Robotic nerve-sparing radical parametrectomy : feasibility and technique .
	manualset3
135635	3	406471	13	NULL	NULL	0	NULL	technique	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Robotic nerve-sparing radical parametrectomy : feasibility and technique .
	manualset3
135636	1	406472	13	NULL	NULL	0	NULL	Robustness 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Robustness of traveling waves in ongoing activity of visual cortex .
	manualset3
135637	2	406472	13	NULL	NULL	0	NULL	waves	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Robustness of traveling waves in ongoing activity of visual cortex .
	manualset3
135638	3	406472	13	NULL	NULL	0	NULL	activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Robustness of traveling waves in ongoing activity of visual cortex .
	manualset3
135639	4	406472	13	NULL	NULL	0	NULL	visual cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Robustness of traveling waves in ongoing activity of visual cortex .
	manualset3
135640	1	406473	13	NULL	NULL	0	NULL	Rod responses 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rod responses were strongly reduced compared with cone responses .
	manualset3
135641	2	406473	13	NULL	NULL	0	NULL	cone responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rod responses were strongly reduced compared with cone responses .
	manualset3
135642	1	406474	13	NULL	NULL	0	NULL	Rodent MATE2 proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Rodent MATE2 proteins are class III MATE transporters , the molecular nature , as well as transport properties , of which remain to be characterized .
	manualset3
135643	2	406474	13	NULL	NULL	0	NULL	class III MATE transporters	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Rodent MATE2 proteins are class III MATE transporters , the molecular nature , as well as transport properties , of which remain to be characterized .
	manualset3
135644	3	406474	13	NULL	NULL	0	NULL	molecular nature	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rodent MATE2 proteins are class III MATE transporters , the molecular nature , as well as transport properties , of which remain to be characterized .
	manualset3
135645	4	406474	13	NULL	NULL	0	NULL	transport properties	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rodent MATE2 proteins are class III MATE transporters , the molecular nature , as well as transport properties , of which remain to be characterized .
	manualset3
135646	1	406475	13	NULL	NULL	0	NULL	Rodin	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Rodin , Patton , Edison , Wilson , Einstein : were they really learning disabled ?
	manualset3
135647	2	406475	13	NULL	NULL	0	NULL	Patton	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Rodin , Patton , Edison , Wilson , Einstein : were they really learning disabled ?
	manualset3
135648	3	406475	13	NULL	NULL	0	NULL	Edison 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Rodin , Patton , Edison , Wilson , Einstein : were they really learning disabled ?
	manualset3
135649	4	406475	13	NULL	NULL	0	NULL	Wilson	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Rodin , Patton , Edison , Wilson , Einstein : were they really learning disabled ?
	manualset3
135650	5	406475	13	NULL	NULL	0	NULL	Einstein	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Rodin , Patton , Edison , Wilson , Einstein : were they really learning disabled ?
	manualset3
135651	1	406476	13	NULL	NULL	0	NULL	Role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role and localization of nucleonic acids of head ) .
	manualset3
135652	2	406476	13	NULL	NULL	0	NULL	localization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role and localization of nucleonic acids of head ) .
	manualset3
135653	3	406476	13	NULL	NULL	0	NULL	nucleonic acids	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Role and localization of nucleonic acids of head ) .
	manualset3
135654	4	406476	13	NULL	NULL	0	NULL	head	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Role and localization of nucleonic acids of head ) .
	manualset3
135655	1	406477	13	NULL	NULL	0	NULL	Role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role for p27 ( Kip1 ) in Vascular Smooth Muscle Cell Migration .
	manualset3
135656	2	406477	13	NULL	NULL	0	NULL	p27 ( Kip1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Role for p27 ( Kip1 ) in Vascular Smooth Muscle Cell Migration .
	manualset3
135657	3	406477	13	NULL	NULL	0	NULL	Vascular Smooth Muscle Cell Migration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role for p27 ( Kip1 ) in Vascular Smooth Muscle Cell Migration .
	manualset3
135658	1	406478	13	NULL	NULL	0	NULL	Role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of CD4 ( + ) and CD8 ( + ) T cells in the prevention of measles virus-induced encephalitis in mice .
	manualset3
135659	2	406478	13	NULL	NULL	0	NULL	CD4 ( + ) T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of CD4 ( + ) and CD8 ( + ) T cells in the prevention of measles virus-induced encephalitis in mice .
	manualset3
135660	3	406478	13	NULL	NULL	0	NULL	CD8 ( + ) T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of CD4 ( + ) and CD8 ( + ) T cells in the prevention of measles virus-induced encephalitis in mice .
	manualset3
135661	4	406478	13	NULL	NULL	0	NULL	prevention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of CD4 ( + ) and CD8 ( + ) T cells in the prevention of measles virus-induced encephalitis in mice .
	manualset3
135662	5	406478	13	NULL	NULL	0	NULL	measles virus-induced encephalitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of CD4 ( + ) and CD8 ( + ) T cells in the prevention of measles virus-induced encephalitis in mice .
	manualset3
135663	6	406478	13	NULL	NULL	0	NULL	mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of CD4 ( + ) and CD8 ( + ) T cells in the prevention of measles virus-induced encephalitis in mice .
	manualset3
135664	1	406479	13	NULL	NULL	0	NULL	Role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of Glu-67 and Arg-368 in the catalytic mechanism .
	manualset3
135665	2	406479	13	NULL	NULL	0	NULL	Glu-67	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of Glu-67 and Arg-368 in the catalytic mechanism .
	manualset3
135666	3	406479	13	NULL	NULL	0	NULL	Arg-368 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of Glu-67 and Arg-368 in the catalytic mechanism .
	manualset3
135667	4	406479	13	NULL	NULL	0	NULL	catalytic mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of Glu-67 and Arg-368 in the catalytic mechanism .
	manualset3
135668	1	406480	13	NULL	NULL	0	NULL	approach	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A new approach to detection of the bregma point on the rat skull .
	manualset3
135669	2	406480	13	NULL	NULL	0	NULL	detection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A new approach to detection of the bregma point on the rat skull .
	manualset3
135670	3	406480	13	NULL	NULL	0	NULL	bregma point	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A new approach to detection of the bregma point on the rat skull .
	manualset3
135671	4	406480	13	NULL	NULL	0	NULL	rat skull	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A new approach to detection of the bregma point on the rat skull .
	manualset3
135672	1	406481	13	NULL	NULL	0	NULL	Role 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of Neural NO Synthase ( nNOS ) Uncoupling in the Dysfunctional Nitrergic Vasorelaxation of Penile Arteries from Insulin-Resistant Obese Zucker Rats .
	manualset3
135673	2	406481	13	NULL	NULL	0	NULL	Neural NO Synthase ( nNOS ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of Neural NO Synthase ( nNOS ) Uncoupling in the Dysfunctional Nitrergic Vasorelaxation of Penile Arteries from Insulin-Resistant Obese Zucker Rats .
	manualset3
135674	3	406481	13	NULL	NULL	0	NULL	Dysfunctional Nitrergic Vasorelaxation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of Neural NO Synthase ( nNOS ) Uncoupling in the Dysfunctional Nitrergic Vasorelaxation of Penile Arteries from Insulin-Resistant Obese Zucker Rats .
	manualset3
135675	4	406481	13	NULL	NULL	0	NULL	Penile Arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of Neural NO Synthase ( nNOS ) Uncoupling in the Dysfunctional Nitrergic Vasorelaxation of Penile Arteries from Insulin-Resistant Obese Zucker Rats .
	manualset3
135676	5	406481	13	NULL	NULL	0	NULL	Insulin-Resistant Obese Zucker Rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of Neural NO Synthase ( nNOS ) Uncoupling in the Dysfunctional Nitrergic Vasorelaxation of Penile Arteries from Insulin-Resistant Obese Zucker Rats .
	manualset3
135677	1	406482	13	NULL	NULL	0	NULL	Role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of PCNA-dependent stimulation of 3 ' - phosphodiesterase and 3 ' -5 ' exonuclease activities of human Ape2 in repair of oxidative DNA damage .
	manualset3
135678	2	406482	13	NULL	NULL	0	NULL	PCNA-dependent stimulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of PCNA-dependent stimulation of 3 ' - phosphodiesterase and 3 ' -5 ' exonuclease activities of human Ape2 in repair of oxidative DNA damage .
	manualset3
135679	3	406482	13	NULL	NULL	0	NULL	3 ' - phosphodiesterase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of PCNA-dependent stimulation of 3 ' - phosphodiesterase and 3 ' -5 ' exonuclease activities of human Ape2 in repair of oxidative DNA damage .
	manualset3
135680	4	406482	13	NULL	NULL	0	NULL	3 ' -5 ' exonuclease activities 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of PCNA-dependent stimulation of 3 ' - phosphodiesterase and 3 ' -5 ' exonuclease activities of human Ape2 in repair of oxidative DNA damage .
	manualset3
135681	5	406482	13	NULL	NULL	0	NULL	human Ape2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of PCNA-dependent stimulation of 3 ' - phosphodiesterase and 3 ' -5 ' exonuclease activities of human Ape2 in repair of oxidative DNA damage .
	manualset3
135682	6	406482	13	NULL	NULL	0	NULL	repair 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of PCNA-dependent stimulation of 3 ' - phosphodiesterase and 3 ' -5 ' exonuclease activities of human Ape2 in repair of oxidative DNA damage .
	manualset3
135683	7	406482	13	NULL	NULL	0	NULL	oxidative DNA damage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of PCNA-dependent stimulation of 3 ' - phosphodiesterase and 3 ' -5 ' exonuclease activities of human Ape2 in repair of oxidative DNA damage .
	manualset3
135684	1	406483	13	NULL	NULL	0	NULL	Role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of SERCA1 truncated isoform in the proapoptotic calcium transfer from ER to mitochondria during ER stress .
	manualset3
135685	2	406483	13	NULL	NULL	0	NULL	SERCA1 truncated isoform	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of SERCA1 truncated isoform in the proapoptotic calcium transfer from ER to mitochondria during ER stress .
	manualset3
135686	3	406483	13	NULL	NULL	0	NULL	proapoptotic calcium transfer	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of SERCA1 truncated isoform in the proapoptotic calcium transfer from ER to mitochondria during ER stress .
	manualset3
135687	4	406483	13	NULL	NULL	0	NULL	ER	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of SERCA1 truncated isoform in the proapoptotic calcium transfer from ER to mitochondria during ER stress .
	manualset3
135688	5	406483	13	NULL	NULL	0	NULL	mitochondria	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of SERCA1 truncated isoform in the proapoptotic calcium transfer from ER to mitochondria during ER stress .
	manualset3
135689	6	406483	13	NULL	NULL	0	NULL	ER stress	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of SERCA1 truncated isoform in the proapoptotic calcium transfer from ER to mitochondria during ER stress .
	manualset3
135690	1	406484	13	NULL	NULL	0	NULL	Role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of a pituitary-specific transcription factor ( pit-1 / GHF-1 ) or a closely related protein in cAMP regulation of human thyrotropin-beta subunit gene expression .
	manualset3
135691	2	406484	13	NULL	NULL	0	NULL	pituitary-specific transcription factor ( pit-1 / GHF-1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of a pituitary-specific transcription factor ( pit-1 / GHF-1 ) or a closely related protein in cAMP regulation of human thyrotropin-beta subunit gene expression .
	manualset3
135692	3	406484	13	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of a pituitary-specific transcription factor ( pit-1 / GHF-1 ) or a closely related protein in cAMP regulation of human thyrotropin-beta subunit gene expression .
	manualset3
135693	4	406484	13	NULL	NULL	0	NULL	cAMP regulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of a pituitary-specific transcription factor ( pit-1 / GHF-1 ) or a closely related protein in cAMP regulation of human thyrotropin-beta subunit gene expression .
	manualset3
135694	5	406484	13	NULL	NULL	0	NULL	human thyrotropin-beta subunit gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of a pituitary-specific transcription factor ( pit-1 / GHF-1 ) or a closely related protein in cAMP regulation of human thyrotropin-beta subunit gene expression .
	manualset3
135695	1	406485	13	NULL	NULL	0	NULL	Role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of agonist and antagonist muscle strength in performance of rapid movements .
	manualset3
135696	2	406485	13	NULL	NULL	0	NULL	agonist muscle strength 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of agonist and antagonist muscle strength in performance of rapid movements .
	manualset3
135697	3	406485	13	NULL	NULL	0	NULL	antagonist muscle strength 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of agonist and antagonist muscle strength in performance of rapid movements .
	manualset3
135698	4	406485	13	NULL	NULL	0	NULL	performance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of agonist and antagonist muscle strength in performance of rapid movements .
	manualset3
135699	5	406485	13	NULL	NULL	0	NULL	rapid movements	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of agonist and antagonist muscle strength in performance of rapid movements .
	manualset3
135700	1	406486	13	NULL	NULL	0	NULL	Role 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of attempted vaginal delivery in the management of placenta previa .
	manualset3
135701	2	406486	13	NULL	NULL	0	NULL	vaginal delivery	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of attempted vaginal delivery in the management of placenta previa .
	manualset3
135702	3	406486	13	NULL	NULL	0	NULL	management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of attempted vaginal delivery in the management of placenta previa .
	manualset3
135703	4	406486	13	NULL	NULL	0	NULL	placenta previa 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of attempted vaginal delivery in the management of placenta previa .
	manualset3
135704	1	406487	13	NULL	NULL	0	NULL	Role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of beta-arrestin 1 in the metastatic progression of colorectal cancer .
	manualset3
135705	2	406487	13	NULL	NULL	0	NULL	beta-arrestin 1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of beta-arrestin 1 in the metastatic progression of colorectal cancer .
	manualset3
135706	3	406487	13	NULL	NULL	0	NULL	metastatic progression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of beta-arrestin 1 in the metastatic progression of colorectal cancer .
	manualset3
135707	4	406487	13	NULL	NULL	0	NULL	colorectal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of beta-arrestin 1 in the metastatic progression of colorectal cancer .
	manualset3
135708	1	406488	13	NULL	NULL	0	NULL	Role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of bone marrow-derived progenitor cells in the maintenance and regeneration of dental mesenchymal tissues .
	manualset3
135709	2	406488	13	NULL	NULL	0	NULL	bone marrow-derived progenitor cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of bone marrow-derived progenitor cells in the maintenance and regeneration of dental mesenchymal tissues .
	manualset3
135710	3	406488	13	NULL	NULL	0	NULL	maintenance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of bone marrow-derived progenitor cells in the maintenance and regeneration of dental mesenchymal tissues .
	manualset3
135711	4	406488	13	NULL	NULL	0	NULL	regeneration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of bone marrow-derived progenitor cells in the maintenance and regeneration of dental mesenchymal tissues .
	manualset3
135712	5	406488	13	NULL	NULL	0	NULL	dental mesenchymal tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of bone marrow-derived progenitor cells in the maintenance and regeneration of dental mesenchymal tissues .
	manualset3
135713	1	406489	13	NULL	NULL	0	NULL	Role 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of cocontraction in arm movement accuracy .
	manualset3
135714	2	406489	13	NULL	NULL	0	NULL	cocontraction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of cocontraction in arm movement accuracy .
	manualset3
135715	3	406489	13	NULL	NULL	0	NULL	arm movement accuracy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of cocontraction in arm movement accuracy .
	manualset3
135716	1	406490	13	NULL	NULL	0	NULL	Role 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of connexin43 and ATP in long-range bystander radiation damage and oncogenesis in vivo .
	manualset3
135717	2	406490	13	NULL	NULL	0	NULL	connexin43	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of connexin43 and ATP in long-range bystander radiation damage and oncogenesis in vivo .
	manualset3
135718	3	406490	13	NULL	NULL	0	NULL	ATP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of connexin43 and ATP in long-range bystander radiation damage and oncogenesis in vivo .
	manualset3
135719	4	406490	13	NULL	NULL	0	NULL	long-range bystander radiation damage 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of connexin43 and ATP in long-range bystander radiation damage and oncogenesis in vivo .
	manualset3
135720	5	406490	13	NULL	NULL	0	NULL	oncogenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of connexin43 and ATP in long-range bystander radiation damage and oncogenesis in vivo .
	manualset3
135815	1	406491	13	NULL	NULL	0	NULL	approach	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A new approach to enhance the natural properties of bark by covalent grafting of oligogalacturonans was developed .
	manualset3
135816	2	406491	13	NULL	NULL	0	NULL	natural properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new approach to enhance the natural properties of bark by covalent grafting of oligogalacturonans was developed .
	manualset3
135817	3	406491	13	NULL	NULL	0	NULL	bark	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A new approach to enhance the natural properties of bark by covalent grafting of oligogalacturonans was developed .
	manualset3
135818	4	406491	13	NULL	NULL	0	NULL	covalent grafting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A new approach to enhance the natural properties of bark by covalent grafting of oligogalacturonans was developed .
	manualset3
135819	5	406491	13	NULL	NULL	0	NULL	oligogalacturonans 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A new approach to enhance the natural properties of bark by covalent grafting of oligogalacturonans was developed .
	manualset3
135820	1	406492	13	NULL	NULL	0	NULL	Role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of cross-linking agents in determining the biochemical and pharmacokinetic properties of Mgr6-clavin immunotoxins .
	manualset3
135821	2	406492	13	NULL	NULL	0	NULL	cross-linking agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of cross-linking agents in determining the biochemical and pharmacokinetic properties of Mgr6-clavin immunotoxins .
	manualset3
135822	3	406492	13	NULL	NULL	0	NULL	biochemical properties 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of cross-linking agents in determining the biochemical and pharmacokinetic properties of Mgr6-clavin immunotoxins .
	manualset3
135823	4	406492	13	NULL	NULL	0	NULL	pharmacokinetic properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of cross-linking agents in determining the biochemical and pharmacokinetic properties of Mgr6-clavin immunotoxins .
	manualset3
135824	5	406492	13	NULL	NULL	0	NULL	Mgr6-clavin immunotoxins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of cross-linking agents in determining the biochemical and pharmacokinetic properties of Mgr6-clavin immunotoxins .
	manualset3
135825	1	406493	13	NULL	NULL	0	NULL	Role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of cytoskeletal organization in the regulation of adenylate cyclase-cyclic adenosine monophosphate by hormones .
	manualset3
135826	2	406493	13	NULL	NULL	0	NULL	cytoskeletal organization 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of cytoskeletal organization in the regulation of adenylate cyclase-cyclic adenosine monophosphate by hormones .
	manualset3
135827	3	406493	13	NULL	NULL	0	NULL	regulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of cytoskeletal organization in the regulation of adenylate cyclase-cyclic adenosine monophosphate by hormones .
	manualset3
135828	4	406493	13	NULL	NULL	0	NULL	adenylate cyclase-cyclic adenosine monophosphate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of cytoskeletal organization in the regulation of adenylate cyclase-cyclic adenosine monophosphate by hormones .
	manualset3
135829	5	406493	13	NULL	NULL	0	NULL	hormones	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of cytoskeletal organization in the regulation of adenylate cyclase-cyclic adenosine monophosphate by hormones .
	manualset3
135830	1	406494	13	NULL	NULL	0	NULL	Role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of glutathione in reduction of arsenate and of gamma-glutamyltranspeptidase in disposition of arsenite in rats .
	manualset3
135831	2	406494	13	NULL	NULL	0	NULL	glutathione	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of glutathione in reduction of arsenate and of gamma-glutamyltranspeptidase in disposition of arsenite in rats .
	manualset3
135832	3	406494	13	NULL	NULL	0	NULL	reduction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of glutathione in reduction of arsenate and of gamma-glutamyltranspeptidase in disposition of arsenite in rats .
	manualset3
135833	4	406494	13	NULL	NULL	0	NULL	arsenate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of glutathione in reduction of arsenate and of gamma-glutamyltranspeptidase in disposition of arsenite in rats .
	manualset3
135834	5	406494	13	NULL	NULL	0	NULL	gamma-glutamyltranspeptidase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of glutathione in reduction of arsenate and of gamma-glutamyltranspeptidase in disposition of arsenite in rats .
	manualset3
135835	6	406494	13	NULL	NULL	0	NULL	disposition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of glutathione in reduction of arsenate and of gamma-glutamyltranspeptidase in disposition of arsenite in rats .
	manualset3
135836	7	406494	13	NULL	NULL	0	NULL	arsenite 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of glutathione in reduction of arsenate and of gamma-glutamyltranspeptidase in disposition of arsenite in rats .
	manualset3
135837	8	406494	13	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of glutathione in reduction of arsenate and of gamma-glutamyltranspeptidase in disposition of arsenite in rats .
	manualset3
135838	1	406495	13	NULL	NULL	0	NULL	Role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of hepcidin in iron metabolism and potential clinical applications .
	manualset3
135839	2	406495	13	NULL	NULL	0	NULL	hepcidin	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of hepcidin in iron metabolism and potential clinical applications .
	manualset3
135840	3	406495	13	NULL	NULL	0	NULL	iron metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of hepcidin in iron metabolism and potential clinical applications .
	manualset3
135841	4	406495	13	NULL	NULL	0	NULL	potential clinical applications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of hepcidin in iron metabolism and potential clinical applications .
	manualset3
135842	1	406496	13	NULL	NULL	0	NULL	Role 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of laparoscopy in the diagnosis and treatment of prostate cancer .
	manualset3
135843	2	406496	13	NULL	NULL	0	NULL	laparoscopy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of laparoscopy in the diagnosis and treatment of prostate cancer .
	manualset3
135844	3	406496	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of laparoscopy in the diagnosis and treatment of prostate cancer .
	manualset3
135845	4	406496	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of laparoscopy in the diagnosis and treatment of prostate cancer .
	manualset3
135846	5	406496	13	NULL	NULL	0	NULL	prostate cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of laparoscopy in the diagnosis and treatment of prostate cancer .
	manualset3
135847	1	406497	13	NULL	NULL	0	NULL	Role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of lipoprotein lipase in lipoprotein metabolism ) .
	manualset3
135848	2	406497	13	NULL	NULL	0	NULL	lipoprotein lipase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of lipoprotein lipase in lipoprotein metabolism ) .
	manualset3
135849	3	406497	13	NULL	NULL	0	NULL	lipoprotein metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of lipoprotein lipase in lipoprotein metabolism ) .
	manualset3
135850	1	406498	13	NULL	NULL	0	NULL	Role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of opioidergic and serotonergic mechanisms in cough and antitussives .
	manualset3
135851	2	406498	13	NULL	NULL	0	NULL	opioidergic mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of opioidergic and serotonergic mechanisms in cough and antitussives .
	manualset3
135852	3	406498	13	NULL	NULL	0	NULL	serotonergic mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of opioidergic and serotonergic mechanisms in cough and antitussives .
	manualset3
135853	4	406498	13	NULL	NULL	0	NULL	cough	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of opioidergic and serotonergic mechanisms in cough and antitussives .
	manualset3
135854	5	406498	13	NULL	NULL	0	NULL	antitussives	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of opioidergic and serotonergic mechanisms in cough and antitussives .
	manualset3
135855	1	406499	13	NULL	NULL	0	NULL	Role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of peripherin/rds in vertebrate photoreceptor architecture and inherited retinal degenerations .
	manualset3
135856	2	406499	13	NULL	NULL	0	NULL	peripherin/rds	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of peripherin/rds in vertebrate photoreceptor architecture and inherited retinal degenerations .
	manualset3
135857	3	406499	13	NULL	NULL	0	NULL	vertebrate photoreceptor architecture	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of peripherin/rds in vertebrate photoreceptor architecture and inherited retinal degenerations .
	manualset3
135858	4	406499	13	NULL	NULL	0	NULL	retinal degenerations 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of peripherin/rds in vertebrate photoreceptor architecture and inherited retinal degenerations .
	manualset3
135859	1	406500	13	NULL	NULL	0	NULL	approach	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A new approach to infants with severe obstructive uropathy : early complete reconstruction .
	manualset3
135860	2	406500	13	NULL	NULL	0	NULL	infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A new approach to infants with severe obstructive uropathy : early complete reconstruction .
	manualset3
135861	3	406500	13	NULL	NULL	0	NULL	severe obstructive uropathy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A new approach to infants with severe obstructive uropathy : early complete reconstruction .
	manualset3
135862	4	406500	13	NULL	NULL	0	NULL	reconstruction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A new approach to infants with severe obstructive uropathy : early complete reconstruction .
	manualset3
135863	1	406501	13	NULL	NULL	0	NULL	Role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of the SaeRS two-component regulatory system in Staphylococcus epidermidis autolysis and biofilm formation .
	manualset3
135864	2	406501	13	NULL	NULL	0	NULL	SaeRS two-component regulatory system	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of the SaeRS two-component regulatory system in Staphylococcus epidermidis autolysis and biofilm formation .
	manualset3
135865	3	406501	13	NULL	NULL	0	NULL	Staphylococcus epidermidis autolysis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of the SaeRS two-component regulatory system in Staphylococcus epidermidis autolysis and biofilm formation .
	manualset3
135866	4	406501	13	NULL	NULL	0	NULL	biofilm formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of the SaeRS two-component regulatory system in Staphylococcus epidermidis autolysis and biofilm formation .
	manualset3
135867	1	406502	13	NULL	NULL	0	NULL	Role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of the U.S. Congress in setting goals and priorities for research on nutrition and aging .
	manualset3
135868	2	406502	13	NULL	NULL	0	NULL	U.S. Congress	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of the U.S. Congress in setting goals and priorities for research on nutrition and aging .
	manualset3
135869	3	406502	13	NULL	NULL	0	NULL	setting goals 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of the U.S. Congress in setting goals and priorities for research on nutrition and aging .
	manualset3
135870	4	406502	13	NULL	NULL	0	NULL	priorities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of the U.S. Congress in setting goals and priorities for research on nutrition and aging .
	manualset3
135871	5	406502	13	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of the U.S. Congress in setting goals and priorities for research on nutrition and aging .
	manualset3
135872	6	406502	13	NULL	NULL	0	NULL	nutrition	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of the U.S. Congress in setting goals and priorities for research on nutrition and aging .
	manualset3
135873	7	406502	13	NULL	NULL	0	NULL	aging	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of the U.S. Congress in setting goals and priorities for research on nutrition and aging .
	manualset3
135874	1	406503	13	NULL	NULL	0	NULL	Role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of ultrasonography in blunt abdominal trauma .
	manualset3
135875	2	406503	13	NULL	NULL	0	NULL	ultrasonography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of ultrasonography in blunt abdominal trauma .
	manualset3
135876	3	406503	13	NULL	NULL	0	NULL	blunt abdominal trauma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of ultrasonography in blunt abdominal trauma .
	manualset3
135877	1	406504	13	NULL	NULL	0	NULL	Roles	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Roles of BOR1 , DUR3 , and FPS1 in boron transport and tolerance in Saccharomyces cerevisiae .
	manualset3
135878	2	406504	13	NULL	NULL	0	NULL	BOR1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Roles of BOR1 , DUR3 , and FPS1 in boron transport and tolerance in Saccharomyces cerevisiae .
	manualset3
135879	3	406504	13	NULL	NULL	0	NULL	DUR3 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Roles of BOR1 , DUR3 , and FPS1 in boron transport and tolerance in Saccharomyces cerevisiae .
	manualset3
135880	4	406504	13	NULL	NULL	0	NULL	FPS1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Roles of BOR1 , DUR3 , and FPS1 in boron transport and tolerance in Saccharomyces cerevisiae .
	manualset3
135881	5	406504	13	NULL	NULL	0	NULL	boron transport	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Roles of BOR1 , DUR3 , and FPS1 in boron transport and tolerance in Saccharomyces cerevisiae .
	manualset3
135882	6	406504	13	NULL	NULL	0	NULL	tolerance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Roles of BOR1 , DUR3 , and FPS1 in boron transport and tolerance in Saccharomyces cerevisiae .
	manualset3
135883	7	406504	13	NULL	NULL	0	NULL	Saccharomyces cerevisiae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Roles of BOR1 , DUR3 , and FPS1 in boron transport and tolerance in Saccharomyces cerevisiae .
	manualset3
135884	1	406505	13	NULL	NULL	0	NULL	Roles	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Roles of the AGE-RAGE system in vascular injury in diabetes .
	manualset3
135885	2	406505	13	NULL	NULL	0	NULL	AGE-RAGE system	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Roles of the AGE-RAGE system in vascular injury in diabetes .
	manualset3
135886	3	406505	13	NULL	NULL	0	NULL	vascular injury 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Roles of the AGE-RAGE system in vascular injury in diabetes .
	manualset3
135887	4	406505	13	NULL	NULL	0	NULL	diabetes 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Roles of the AGE-RAGE system in vascular injury in diabetes .
	manualset3
135888	1	406506	13	NULL	NULL	0	NULL	Root-surface caries	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Root-surface caries , like enamel caries , develops as a subsurface type of mineral loss .
	manualset3
135889	2	406506	13	NULL	NULL	0	NULL	enamel caries	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Root-surface caries , like enamel caries , develops as a subsurface type of mineral loss .
	manualset3
135890	3	406506	13	NULL	NULL	0	NULL	subsurface type of mineral loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Root-surface caries , like enamel caries , develops as a subsurface type of mineral loss .
	manualset3
135891	1	406507	13	NULL	NULL	0	NULL	Rooted plantlets 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rooted plantlets were able to grow in soil after a short period of acclimatization .
	manualset3
135892	2	406507	13	NULL	NULL	0	NULL	soil 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Rooted plantlets were able to grow in soil after a short period of acclimatization .
	manualset3
135893	3	406507	13	NULL	NULL	0	NULL	short period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Rooted plantlets were able to grow in soil after a short period of acclimatization .
	manualset3
135894	4	406507	13	NULL	NULL	0	NULL	acclimatization  	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rooted plantlets were able to grow in soil after a short period of acclimatization .
	manualset3
135895	1	406508	13	NULL	NULL	0	NULL	aspect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A new aspect of aminoglycoside ototoxicity : impairment of cochlear dopamine release .
	manualset3
135896	2	406508	13	NULL	NULL	0	NULL	aminoglycoside ototoxicity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A new aspect of aminoglycoside ototoxicity : impairment of cochlear dopamine release .
	manualset3
135897	3	406508	13	NULL	NULL	0	NULL	impairment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A new aspect of aminoglycoside ototoxicity : impairment of cochlear dopamine release .
	manualset3
135898	4	406508	13	NULL	NULL	0	NULL	cochlear dopamine release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A new aspect of aminoglycoside ototoxicity : impairment of cochlear dopamine release .
	manualset3
135899	1	406509	13	NULL	NULL	0	NULL	Rostral area 12r 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Rostral area 12r displayed connections mostly with rostral prefrontal and orbitofrontal areas and relatively weaker connections with the fundus and the upper bank of the superior temporal sulcus .
	manualset3
135900	2	406509	13	NULL	NULL	0	NULL	connections	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rostral area 12r displayed connections mostly with rostral prefrontal and orbitofrontal areas and relatively weaker connections with the fundus and the upper bank of the superior temporal sulcus .
	manualset3
135901	3	406509	13	NULL	NULL	0	NULL	rostral prefrontal areas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Rostral area 12r displayed connections mostly with rostral prefrontal and orbitofrontal areas and relatively weaker connections with the fundus and the upper bank of the superior temporal sulcus .
	manualset3
135902	4	406509	13	NULL	NULL	0	NULL	orbitofrontal areas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Rostral area 12r displayed connections mostly with rostral prefrontal and orbitofrontal areas and relatively weaker connections with the fundus and the upper bank of the superior temporal sulcus .
	manualset3
135903	5	406509	13	NULL	NULL	0	NULL	connections	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rostral area 12r displayed connections mostly with rostral prefrontal and orbitofrontal areas and relatively weaker connections with the fundus and the upper bank of the superior temporal sulcus .
	manualset3
135904	6	406509	13	NULL	NULL	0	NULL	fundus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Rostral area 12r displayed connections mostly with rostral prefrontal and orbitofrontal areas and relatively weaker connections with the fundus and the upper bank of the superior temporal sulcus .
	manualset3
135905	7	406509	13	NULL	NULL	0	NULL	upper bank 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Rostral area 12r displayed connections mostly with rostral prefrontal and orbitofrontal areas and relatively weaker connections with the fundus and the upper bank of the superior temporal sulcus .
	manualset3
135906	8	406509	13	NULL	NULL	0	NULL	superior temporal sulcus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Rostral area 12r displayed connections mostly with rostral prefrontal and orbitofrontal areas and relatively weaker connections with the fundus and the upper bank of the superior temporal sulcus .
	manualset3
135907	1	406510	13	NULL	NULL	0	NULL	Rotation-invariant image	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Rotation-invariant image and video description with local binary pattern features .
	manualset3
135908	2	406510	13	NULL	NULL	0	NULL	video description 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rotation-invariant image and video description with local binary pattern features .
	manualset3
135909	3	406510	13	NULL	NULL	0	NULL	local binary pattern features	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rotation-invariant image and video description with local binary pattern features .
	manualset3
135911	1	406511	13	NULL	NULL	0	NULL	Rotational relaxation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rotational relaxation is faster in o-D ( 2 ) than in p-H ( 2 ) and faster in p-H ( 2 ) than in Ne .
	manualset3
135915	2	406511	13	NULL	NULL	0	NULL	o-D ( 2 )	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Rotational relaxation is faster in o-D ( 2 ) than in p-H ( 2 ) and faster in p-H ( 2 ) than in Ne .
	manualset3
135917	3	406511	13	NULL	NULL	0	NULL	p-H ( 2 ) 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Rotational relaxation is faster in o-D ( 2 ) than in p-H ( 2 ) and faster in p-H ( 2 ) than in Ne .
	manualset3
135919	4	406511	13	NULL	NULL	0	NULL	p-H ( 2 )	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Rotational relaxation is faster in o-D ( 2 ) than in p-H ( 2 ) and faster in p-H ( 2 ) than in Ne .
	manualset3
135920	5	406511	13	NULL	NULL	0	NULL	Ne	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Rotational relaxation is faster in o-D ( 2 ) than in p-H ( 2 ) and faster in p-H ( 2 ) than in Ne .
	manualset3
135923	1	406512	13	NULL	NULL	0	NULL	Rottlerin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rottlerin blocked c-Abl activation , but the c-Abl inhibitor STI-571 increased MGO and cisplatin-induced apoptosis by 50 % .
	manualset3
135924	2	406512	13	NULL	NULL	0	NULL	c-Abl 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Rottlerin blocked c-Abl activation , but the c-Abl inhibitor STI-571 increased MGO and cisplatin-induced apoptosis by 50 % .
	manualset3
135925	3	406512	13	NULL	NULL	0	NULL	activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rottlerin blocked c-Abl activation , but the c-Abl inhibitor STI-571 increased MGO and cisplatin-induced apoptosis by 50 % .
	manualset3
135926	4	406512	13	NULL	NULL	0	NULL	c-Abl inhibitor STI-571	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rottlerin blocked c-Abl activation , but the c-Abl inhibitor STI-571 increased MGO and cisplatin-induced apoptosis by 50 % .
	manualset3
135927	5	406512	13	NULL	NULL	0	NULL	MGO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rottlerin blocked c-Abl activation , but the c-Abl inhibitor STI-571 increased MGO and cisplatin-induced apoptosis by 50 % .
	manualset3
135928	6	406512	13	NULL	NULL	0	NULL	cisplatin-induced apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rottlerin blocked c-Abl activation , but the c-Abl inhibitor STI-571 increased MGO and cisplatin-induced apoptosis by 50 % .
	manualset3
135929	7	406512	13	NULL	NULL	0	NULL	50 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Rottlerin blocked c-Abl activation , but the c-Abl inhibitor STI-571 increased MGO and cisplatin-induced apoptosis by 50 % .
	manualset3
135930	1	406513	13	NULL	NULL	0	NULL	Roughness parameters	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Roughness parameters of teeth that had been scaled and root planed were determined from AFM images acquired both before and after treatment with EDTA .
	manualset3
135931	2	406513	13	NULL	NULL	0	NULL	teeth	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Roughness parameters of teeth that had been scaled and root planed were determined from AFM images acquired both before and after treatment with EDTA .
	manualset3
135932	3	406513	13	NULL	NULL	0	NULL	AFM images	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Roughness parameters of teeth that had been scaled and root planed were determined from AFM images acquired both before and after treatment with EDTA .
	manualset3
135933	4	406513	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Roughness parameters of teeth that had been scaled and root planed were determined from AFM images acquired both before and after treatment with EDTA .
	manualset3
135934	5	406513	13	NULL	NULL	0	NULL	EDTA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Roughness parameters of teeth that had been scaled and root planed were determined from AFM images acquired both before and after treatment with EDTA .
	manualset3
138436	6	406513	13	NULL	NULL	0	NULL	root 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Roughness parameters of teeth that had been scaled and root planed were determined from AFM images acquired both before and after treatment with EDTA .
	manualset3
135935	1	406514	13	NULL	NULL	0	NULL	Case 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Case of a chyliferous mesenteric cyst ) .
	manualset3
135936	2	406514	13	NULL	NULL	0	NULL	chyliferous mesenteric cyst 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Case of a chyliferous mesenteric cyst ) .
	manualset3
135937	1	406515	13	NULL	NULL	0	NULL	assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new assay for the total dopamine receptor-blocking activity of the plasma correlated highly at lower levels with the sum of drug plus metabolites obtained by GLC , but exceeded the sum at higher values .
	manualset3
135938	2	406515	13	NULL	NULL	0	NULL	dopamine receptor-blocking activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A new assay for the total dopamine receptor-blocking activity of the plasma correlated highly at lower levels with the sum of drug plus metabolites obtained by GLC , but exceeded the sum at higher values .
	manualset3
136193	3	406515	13	NULL	NULL	0	NULL	plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A new assay for the total dopamine receptor-blocking activity of the plasma correlated highly at lower levels with the sum of drug plus metabolites obtained by GLC , but exceeded the sum at higher values .
	manualset3
136196	4	406515	13	NULL	NULL	0	NULL	levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A new assay for the total dopamine receptor-blocking activity of the plasma correlated highly at lower levels with the sum of drug plus metabolites obtained by GLC , but exceeded the sum at higher values .
	manualset3
136198	5	406515	13	NULL	NULL	0	NULL	drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A new assay for the total dopamine receptor-blocking activity of the plasma correlated highly at lower levels with the sum of drug plus metabolites obtained by GLC , but exceeded the sum at higher values .
	manualset3
136199	6	406515	13	NULL	NULL	0	NULL	metabolites 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A new assay for the total dopamine receptor-blocking activity of the plasma correlated highly at lower levels with the sum of drug plus metabolites obtained by GLC , but exceeded the sum at higher values .
	manualset3
136202	7	406515	13	NULL	NULL	0	NULL	GLC	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new assay for the total dopamine receptor-blocking activity of the plasma correlated highly at lower levels with the sum of drug plus metabolites obtained by GLC , but exceeded the sum at higher values .
	manualset3
136204	8	406515	13	NULL	NULL	0	NULL	sum	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A new assay for the total dopamine receptor-blocking activity of the plasma correlated highly at lower levels with the sum of drug plus metabolites obtained by GLC , but exceeded the sum at higher values .
	manualset3
136206	9	406515	13	NULL	NULL	0	NULL	values 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A new assay for the total dopamine receptor-blocking activity of the plasma correlated highly at lower levels with the sum of drug plus metabolites obtained by GLC , but exceeded the sum at higher values .
	manualset3
136215	1	406516	13	NULL	NULL	0	NULL	Routes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Routes are presented for synthesizing nano - and mesostructured - tin particles in the form of monocrystalline spheres , cubes , and bars , as well as polycrystalline rods and needles , by the decomposition of decamethylstannocene in organic solvents under various conditions .
	manualset3
136217	2	406516	13	NULL	NULL	0	NULL	nano -tin particles 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Routes are presented for synthesizing nano - and mesostructured - tin particles in the form of monocrystalline spheres , cubes , and bars , as well as polycrystalline rods and needles , by the decomposition of decamethylstannocene in organic solvents under various conditions .
	manualset3
136219	3	406516	13	NULL	NULL	0	NULL	mesostructured - tin particles	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Routes are presented for synthesizing nano - and mesostructured - tin particles in the form of monocrystalline spheres , cubes , and bars , as well as polycrystalline rods and needles , by the decomposition of decamethylstannocene in organic solvents under various conditions .
	manualset3
136220	4	406516	13	NULL	NULL	NULL	NULL	form 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Routes are presented for synthesizing nano - and mesostructured - tin particles in the form of monocrystalline spheres , cubes , and bars , as well as polycrystalline rods and needles , by the decomposition of decamethylstannocene in organic solvents under various conditions .
	manualset3
136223	5	406516	13	NULL	NULL	0	NULL	monocrystalline spheres	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Routes are presented for synthesizing nano - and mesostructured - tin particles in the form of monocrystalline spheres , cubes , and bars , as well as polycrystalline rods and needles , by the decomposition of decamethylstannocene in organic solvents under various conditions .
	manualset3
136225	6	406516	13	NULL	NULL	0	NULL	monocrystalline cubes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Routes are presented for synthesizing nano - and mesostructured - tin particles in the form of monocrystalline spheres , cubes , and bars , as well as polycrystalline rods and needles , by the decomposition of decamethylstannocene in organic solvents under various conditions .
	manualset3
136227	7	406516	13	NULL	NULL	0	NULL	monocrystalline bars	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Routes are presented for synthesizing nano - and mesostructured - tin particles in the form of monocrystalline spheres , cubes , and bars , as well as polycrystalline rods and needles , by the decomposition of decamethylstannocene in organic solvents under various conditions .
	manualset3
136228	8	406516	13	NULL	NULL	0	NULL	polycrystalline rods	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Routes are presented for synthesizing nano - and mesostructured - tin particles in the form of monocrystalline spheres , cubes , and bars , as well as polycrystalline rods and needles , by the decomposition of decamethylstannocene in organic solvents under various conditions .
	manualset3
136230	9	406516	13	NULL	NULL	0	NULL	polycrystalline needles	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Routes are presented for synthesizing nano - and mesostructured - tin particles in the form of monocrystalline spheres , cubes , and bars , as well as polycrystalline rods and needles , by the decomposition of decamethylstannocene in organic solvents under various conditions .
	manualset3
136232	10	406516	13	NULL	NULL	0	NULL	decomposition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Routes are presented for synthesizing nano - and mesostructured - tin particles in the form of monocrystalline spheres , cubes , and bars , as well as polycrystalline rods and needles , by the decomposition of decamethylstannocene in organic solvents under various conditions .
	manualset3
136234	11	406516	13	NULL	NULL	0	NULL	decamethylstannocene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Routes are presented for synthesizing nano - and mesostructured - tin particles in the form of monocrystalline spheres , cubes , and bars , as well as polycrystalline rods and needles , by the decomposition of decamethylstannocene in organic solvents under various conditions .
	manualset3
136237	12	406516	13	NULL	NULL	0	NULL	organic solvents 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Routes are presented for synthesizing nano - and mesostructured - tin particles in the form of monocrystalline spheres , cubes , and bars , as well as polycrystalline rods and needles , by the decomposition of decamethylstannocene in organic solvents under various conditions .
	manualset3
136239	13	406516	13	NULL	NULL	0	NULL	conditions 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Routes are presented for synthesizing nano - and mesostructured - tin particles in the form of monocrystalline spheres , cubes , and bars , as well as polycrystalline rods and needles , by the decomposition of decamethylstannocene in organic solvents under various conditions .
	manualset3
136241	1	406517	13	NULL	NULL	0	NULL	Routine cleft closure 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Routine cleft closure in repair of complete atrioventricular septal defects .
	manualset3
136242	2	406517	13	NULL	NULL	0	NULL	repair	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Routine cleft closure in repair of complete atrioventricular septal defects .
	manualset3
136243	3	406517	13	NULL	NULL	0	NULL	complete atrioventricular septal defects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Routine cleft closure in repair of complete atrioventricular septal defects .
	manualset3
136270	1	406518	13	NULL	NULL	0	NULL	Routine sperm-function tests 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Routine sperm-function tests are warranted to monitor the sperm quality after varicocelectomy and consequent improvement in the outcomes of assisted reproductive technology .
	manualset3
136346	2	406518	13	NULL	NULL	0	NULL	monitor 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Routine sperm-function tests are warranted to monitor the sperm quality after varicocelectomy and consequent improvement in the outcomes of assisted reproductive technology .
	manualset3
136348	3	406518	13	NULL	NULL	0	NULL	sperm quality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Routine sperm-function tests are warranted to monitor the sperm quality after varicocelectomy and consequent improvement in the outcomes of assisted reproductive technology .
	manualset3
136350	4	406518	13	NULL	NULL	0	NULL	varicocelectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Routine sperm-function tests are warranted to monitor the sperm quality after varicocelectomy and consequent improvement in the outcomes of assisted reproductive technology .
	manualset3
136352	5	406518	13	NULL	NULL	0	NULL	improvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Routine sperm-function tests are warranted to monitor the sperm quality after varicocelectomy and consequent improvement in the outcomes of assisted reproductive technology .
	manualset3
136353	6	406518	13	NULL	NULL	0	NULL	outcomes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Routine sperm-function tests are warranted to monitor the sperm quality after varicocelectomy and consequent improvement in the outcomes of assisted reproductive technology .
	manualset3
136355	7	406518	13	NULL	NULL	0	NULL	assisted reproductive technology 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Routine sperm-function tests are warranted to monitor the sperm quality after varicocelectomy and consequent improvement in the outcomes of assisted reproductive technology .
	manualset3
136379	1	406519	13	NULL	NULL	0	NULL	Roxatidine acetate	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Roxatidine acetate , a new H2 receptor antagonist , was compared with ranitidine in the treatment of duodenal ulcers in a double-blind multicentre study .
	manualset3
136380	2	406519	13	NULL	NULL	0	NULL	H2 receptor antagonist 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Roxatidine acetate , a new H2 receptor antagonist , was compared with ranitidine in the treatment of duodenal ulcers in a double-blind multicentre study .
	manualset3
136381	3	406519	13	NULL	NULL	0	NULL	ranitidine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Roxatidine acetate , a new H2 receptor antagonist , was compared with ranitidine in the treatment of duodenal ulcers in a double-blind multicentre study .
	manualset3
136382	4	406519	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Roxatidine acetate , a new H2 receptor antagonist , was compared with ranitidine in the treatment of duodenal ulcers in a double-blind multicentre study .
	manualset3
136383	5	406519	13	NULL	NULL	0	NULL	duodenal ulcers	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Roxatidine acetate , a new H2 receptor antagonist , was compared with ranitidine in the treatment of duodenal ulcers in a double-blind multicentre study .
	manualset3
136384	6	406519	13	NULL	NULL	0	NULL	double-blind multicentre study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Roxatidine acetate , a new H2 receptor antagonist , was compared with ranitidine in the treatment of duodenal ulcers in a double-blind multicentre study .
	manualset3
136385	1	406520	13	NULL	NULL	0	NULL	Rtr1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Rtr1 is a CTD phosphatase that regulates RNA polymerase II during the transition from serine 5 to serine 2 phosphorylation .
	manualset3
136386	2	406520	13	NULL	NULL	0	NULL	CTD phosphatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Rtr1 is a CTD phosphatase that regulates RNA polymerase II during the transition from serine 5 to serine 2 phosphorylation .
	manualset3
136387	3	406520	13	NULL	NULL	0	NULL	RNA polymerase II 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Rtr1 is a CTD phosphatase that regulates RNA polymerase II during the transition from serine 5 to serine 2 phosphorylation .
	manualset3
136388	4	406520	13	NULL	NULL	0	NULL	transition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rtr1 is a CTD phosphatase that regulates RNA polymerase II during the transition from serine 5 to serine 2 phosphorylation .
	manualset3
136389	5	406520	13	NULL	NULL	0	NULL	serine 5	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Rtr1 is a CTD phosphatase that regulates RNA polymerase II during the transition from serine 5 to serine 2 phosphorylation .
	manualset3
136390	6	406520	13	NULL	NULL	0	NULL	serine 2	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Rtr1 is a CTD phosphatase that regulates RNA polymerase II during the transition from serine 5 to serine 2 phosphorylation .
	manualset3
136391	7	406520	13	NULL	NULL	0	NULL	phosphorylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rtr1 is a CTD phosphatase that regulates RNA polymerase II during the transition from serine 5 to serine 2 phosphorylation .
	manualset3
136392	1	406521	13	NULL	NULL	0	NULL	assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new assay of respiratory nitrite reductase was developed in this study .
	manualset3
136393	2	406521	13	NULL	NULL	0	NULL	respiratory nitrite reductase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A new assay of respiratory nitrite reductase was developed in this study .
	manualset3
136394	3	406521	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new assay of respiratory nitrite reductase was developed in this study .
	manualset3
136395	1	406522	13	NULL	NULL	0	NULL	Ruptured proximal lenticulostriate artery fusiform aneurysm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ruptured proximal lenticulostriate artery fusiform aneurysm presenting with subarachnoid hemorrhage : case report .
	manualset3
136396	2	406522	13	NULL	NULL	0	NULL	subarachnoid hemorrhage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ruptured proximal lenticulostriate artery fusiform aneurysm presenting with subarachnoid hemorrhage : case report .
	manualset3
136397	3	406522	13	NULL	NULL	0	NULL	case report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Ruptured proximal lenticulostriate artery fusiform aneurysm presenting with subarachnoid hemorrhage : case report .
	manualset3
136398	1	406523	13	NULL	NULL	0	NULL	Rush	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rush and inadequate operations in primary surgical treatment of the wound , in particular , can cause an additional and severe trauma of the nerve , which repairing proves to be difficult and sometimes even impossible .
	manualset3
136399	2	406523	13	NULL	NULL	0	NULL	inadequate operations 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Rush and inadequate operations in primary surgical treatment of the wound , in particular , can cause an additional and severe trauma of the nerve , which repairing proves to be difficult and sometimes even impossible .
	manualset3
136400	3	406523	13	NULL	NULL	0	NULL	primary surgical treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Rush and inadequate operations in primary surgical treatment of the wound , in particular , can cause an additional and severe trauma of the nerve , which repairing proves to be difficult and sometimes even impossible .
	manualset3
136401	4	406523	13	NULL	NULL	0	NULL	wound	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rush and inadequate operations in primary surgical treatment of the wound , in particular , can cause an additional and severe trauma of the nerve , which repairing proves to be difficult and sometimes even impossible .
	manualset3
136402	5	406523	13	NULL	NULL	0	NULL	severe trauma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rush and inadequate operations in primary surgical treatment of the wound , in particular , can cause an additional and severe trauma of the nerve , which repairing proves to be difficult and sometimes even impossible .
	manualset3
136403	6	406523	13	NULL	NULL	0	NULL	nerve	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Rush and inadequate operations in primary surgical treatment of the wound , in particular , can cause an additional and severe trauma of the nerve , which repairing proves to be difficult and sometimes even impossible .
	manualset3
138437	7	406523	13	NULL	NULL	0	NULL	repairing 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Rush and inadequate operations in primary surgical treatment of the wound , in particular , can cause an additional and severe trauma of the nerve , which repairing proves to be difficult and sometimes even impossible .
	manualset3
136405	1	406524	13	NULL	NULL	NULL	NULL	Ruthenium ( II ) polypyridyl complexes 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ruthenium ( II ) polypyridyl complexes and DNA-from structural probes to cellular imaging and therapeutics .
	manualset3
136414	2	406524	13	NULL	NULL	0	NULL	DNA-from structural probes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Ruthenium ( II ) polypyridyl complexes and DNA-from structural probes to cellular imaging and therapeutics .
	manualset3
136415	3	406524	13	NULL	NULL	0	NULL	cellular imaging 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ruthenium ( II ) polypyridyl complexes and DNA-from structural probes to cellular imaging and therapeutics .
	manualset3
136416	4	406524	13	NULL	NULL	0	NULL	 therapeutics	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ruthenium ( II ) polypyridyl complexes and DNA-from structural probes to cellular imaging and therapeutics .
	manualset3
136417	1	406525	13	NULL	NULL	0	NULL	RyR1 residues Leu922-Asp1112	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	RyR1 residues Leu922-Asp1112 bound specifically to the DHPR II-III loop column , but the corresponding fragment from the cardiac ryanodine receptor ( RyR2 ) did not .
	manualset3
136418	2	406525	13	NULL	NULL	NULL	NULL	DHPR II-III loop column	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	RyR1 residues Leu922-Asp1112 bound specifically to the DHPR II-III loop column , but the corresponding fragment from the cardiac ryanodine receptor ( RyR2 ) did not .
	manualset3
136429	3	406525	13	NULL	NULL	0	NULL	fragment	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	RyR1 residues Leu922-Asp1112 bound specifically to the DHPR II-III loop column , but the corresponding fragment from the cardiac ryanodine receptor ( RyR2 ) did not .
	manualset3
136431	4	406525	13	NULL	NULL	0	NULL	cardiac ryanodine receptor ( RyR2 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	RyR1 residues Leu922-Asp1112 bound specifically to the DHPR II-III loop column , but the corresponding fragment from the cardiac ryanodine receptor ( RyR2 ) did not .
	manualset3
136434	1	406526	13	NULL	NULL	0	NULL	S-1	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	S-1 was administered orally ( 40 mg m ( -2 ) b.i.d. ) for 28 days , followed by a 14-day rest period .
	manualset3
136436	2	406526	13	NULL	NULL	0	NULL	40 mg m ( -2 ) b.i.d	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	S-1 was administered orally ( 40 mg m ( -2 ) b.i.d. ) for 28 days , followed by a 14-day rest period .
	manualset3
136437	3	406526	13	NULL	NULL	0	NULL	28 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	S-1 was administered orally ( 40 mg m ( -2 ) b.i.d. ) for 28 days , followed by a 14-day rest period .
	manualset3
136438	4	406526	13	NULL	NULL	0	NULL	14-day rest period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	S-1 was administered orally ( 40 mg m ( -2 ) b.i.d. ) for 28 days , followed by a 14-day rest period .
	manualset3
136452	1	406527	13	NULL	NULL	0	NULL	S-Adenosyl-L-methionine decarboxylase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	S-Adenosyl-L-methionine decarboxylase ( AdoMetDC ; EC 4.1.1.50 ) is one of the key regulatory enzymes in the biosynthesis of polyamines .
	manualset3
136454	2	406527	13	NULL	NULL	0	NULL	AdoMetDC	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	S-Adenosyl-L-methionine decarboxylase ( AdoMetDC ; EC 4.1.1.50 ) is one of the key regulatory enzymes in the biosynthesis of polyamines .
	manualset3
136457	3	406527	13	NULL	NULL	0	NULL	EC 4.1.1.50 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	S-Adenosyl-L-methionine decarboxylase ( AdoMetDC ; EC 4.1.1.50 ) is one of the key regulatory enzymes in the biosynthesis of polyamines .
	manualset3
136464	4	406527	13	NULL	NULL	0	NULL	key regulatory enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	S-Adenosyl-L-methionine decarboxylase ( AdoMetDC ; EC 4.1.1.50 ) is one of the key regulatory enzymes in the biosynthesis of polyamines .
	manualset3
136465	5	406527	13	NULL	NULL	0	NULL	biosynthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	S-Adenosyl-L-methionine decarboxylase ( AdoMetDC ; EC 4.1.1.50 ) is one of the key regulatory enzymes in the biosynthesis of polyamines .
	manualset3
136466	6	406527	13	NULL	NULL	0	NULL	polyamines 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	S-Adenosyl-L-methionine decarboxylase ( AdoMetDC ; EC 4.1.1.50 ) is one of the key regulatory enzymes in the biosynthesis of polyamines .
	manualset3
136485	1	406528	13	NULL	NULL	0	NULL	S-Glutathionylation ( thiolation ) 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	S-Glutathionylation ( thiolation ) is a ubiquitous redox-sensitive and reversible modification of protein cysteinyl residues that can directly regulate their activity .
	manualset3
136488	2	406528	13	NULL	NULL	0	NULL	modification	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	S-Glutathionylation ( thiolation ) is a ubiquitous redox-sensitive and reversible modification of protein cysteinyl residues that can directly regulate their activity .
	manualset3
136489	3	406528	13	NULL	NULL	0	NULL	protein cysteinyl residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	S-Glutathionylation ( thiolation ) is a ubiquitous redox-sensitive and reversible modification of protein cysteinyl residues that can directly regulate their activity .
	manualset3
136491	4	406528	13	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	S-Glutathionylation ( thiolation ) is a ubiquitous redox-sensitive and reversible modification of protein cysteinyl residues that can directly regulate their activity .
	manualset3
136493	1	406529	13	NULL	NULL	0	NULL	S-allyl-L-cysteine sulfoxide 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	S-allyl-L-cysteine sulfoxide inhibits tumor necrosis factor-alpha induced monocyte adhesion and intercellular cell adhesion molecule-1 expression in human umbilical vein endothelial cells .
	manualset3
136495	2	406529	13	NULL	NULL	0	NULL	tumor necrosis factor-alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	S-allyl-L-cysteine sulfoxide inhibits tumor necrosis factor-alpha induced monocyte adhesion and intercellular cell adhesion molecule-1 expression in human umbilical vein endothelial cells .
	manualset3
136496	3	406529	13	NULL	NULL	0	NULL	monocyte adhesion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	S-allyl-L-cysteine sulfoxide inhibits tumor necrosis factor-alpha induced monocyte adhesion and intercellular cell adhesion molecule-1 expression in human umbilical vein endothelial cells .
	manualset3
136499	4	406529	13	NULL	NULL	0	NULL	intercellular cell adhesion molecule-1 expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	S-allyl-L-cysteine sulfoxide inhibits tumor necrosis factor-alpha induced monocyte adhesion and intercellular cell adhesion molecule-1 expression in human umbilical vein endothelial cells .
	manualset3
136500	5	406529	13	NULL	NULL	0	NULL	human umbilical vein endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	S-allyl-L-cysteine sulfoxide inhibits tumor necrosis factor-alpha induced monocyte adhesion and intercellular cell adhesion molecule-1 expression in human umbilical vein endothelial cells .
	manualset3
136512	1	406530	13	NULL	NULL	0	NULL	assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new assay that detects antibodies to citrullinated peptides , called the anti-CCP assay , has demonstrated a comparable sensitivity but a much higher specificity than the RF test .
	manualset3
136514	2	406530	13	NULL	NULL	0	NULL	antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A new assay that detects antibodies to citrullinated peptides , called the anti-CCP assay , has demonstrated a comparable sensitivity but a much higher specificity than the RF test .
	manualset3
136515	3	406530	13	NULL	NULL	0	NULL	citrullinated peptides 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	A new assay that detects antibodies to citrullinated peptides , called the anti-CCP assay , has demonstrated a comparable sensitivity but a much higher specificity than the RF test .
	manualset3
136516	4	406530	13	NULL	NULL	0	NULL	anti-CCP assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new assay that detects antibodies to citrullinated peptides , called the anti-CCP assay , has demonstrated a comparable sensitivity but a much higher specificity than the RF test .
	manualset3
136518	5	406530	13	NULL	NULL	0	NULL	sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A new assay that detects antibodies to citrullinated peptides , called the anti-CCP assay , has demonstrated a comparable sensitivity but a much higher specificity than the RF test .
	manualset3
136519	6	406530	13	NULL	NULL	0	NULL	specificity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A new assay that detects antibodies to citrullinated peptides , called the anti-CCP assay , has demonstrated a comparable sensitivity but a much higher specificity than the RF test .
	manualset3
136520	7	406530	13	NULL	NULL	0	NULL	RF test 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new assay that detects antibodies to citrullinated peptides , called the anti-CCP assay , has demonstrated a comparable sensitivity but a much higher specificity than the RF test .
	manualset3
131229	1	406531	5	NULL	NULL	0	NULL	S. cerevisiae growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	S. cerevisiae growth and responses to different treatments were monitored by two-dimensional fluorescence spectroscopy , which simultaneously detects the fluorescence of a number of cells ' own fluorophores .
	manualset3
131230	2	406531	5	NULL	NULL	0	NULL	responses 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	S. cerevisiae growth and responses to different treatments were monitored by two-dimensional fluorescence spectroscopy , which simultaneously detects the fluorescence of a number of cells ' own fluorophores .
	manualset3
131231	3	406531	5	NULL	NULL	0	NULL	treatments 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	S. cerevisiae growth and responses to different treatments were monitored by two-dimensional fluorescence spectroscopy , which simultaneously detects the fluorescence of a number of cells ' own fluorophores .
	manualset3
131232	4	406531	5	NULL	NULL	0	NULL	two-dimensional fluorescence spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	S. cerevisiae growth and responses to different treatments were monitored by two-dimensional fluorescence spectroscopy , which simultaneously detects the fluorescence of a number of cells ' own fluorophores .
	manualset3
131233	5	406531	5	NULL	NULL	0	NULL	fluorescence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	S. cerevisiae growth and responses to different treatments were monitored by two-dimensional fluorescence spectroscopy , which simultaneously detects the fluorescence of a number of cells ' own fluorophores .
	manualset3
131234	6	406531	5	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	S. cerevisiae growth and responses to different treatments were monitored by two-dimensional fluorescence spectroscopy , which simultaneously detects the fluorescence of a number of cells ' own fluorophores .
	manualset3
131235	7	406531	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	S. cerevisiae growth and responses to different treatments were monitored by two-dimensional fluorescence spectroscopy , which simultaneously detects the fluorescence of a number of cells ' own fluorophores .
	manualset3
131236	8	406531	5	NULL	NULL	0	NULL	fluorophores 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	S. cerevisiae growth and responses to different treatments were monitored by two-dimensional fluorescence spectroscopy , which simultaneously detects the fluorescence of a number of cells ' own fluorophores .
	manualset3
131237	1	406532	5	NULL	NULL	0	NULL	S. pyogenes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	S. pyogenes , as the other beta-hemolytic streptococci studied remained fully susceptible to beta-lactam antibiotics .
	manualset3
131238	2	406532	5	NULL	NULL	0	NULL	beta-hemolytic streptococci	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	S. pyogenes , as the other beta-hemolytic streptococci studied remained fully susceptible to beta-lactam antibiotics .
	manualset3
131239	3	406532	5	NULL	NULL	0	NULL	beta-lactam antibiotics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	S. pyogenes , as the other beta-hemolytic streptococci studied remained fully susceptible to beta-lactam antibiotics .
	manualset3
131240	1	406533	5	NULL	NULL	0	NULL	S100A8/A9	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	S100A8/A9 , a key mediator for positive feedback growth stimulation of normal human keratinocytes .
	manualset3
131241	2	406533	5	NULL	NULL	0	NULL	key mediator	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	S100A8/A9 , a key mediator for positive feedback growth stimulation of normal human keratinocytes .
	manualset3
131242	3	406533	5	NULL	NULL	0	NULL	 positive feedback growth stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	S100A8/A9 , a key mediator for positive feedback growth stimulation of normal human keratinocytes .
	manualset3
131243	4	406533	5	NULL	NULL	0	NULL	normal human keratinocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	S100A8/A9 , a key mediator for positive feedback growth stimulation of normal human keratinocytes .
	manualset3
131244	1	406534	5	NULL	NULL	0	NULL	SAT 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	SAT was reversibly inactivated on cooling to 0 degrees C. Ultracentrifugal analysis showed that SAT ( a hexamer ) was dissociated mostly into two trimers on cooling to 0 degrees C in the absence of OASS , while in the presence of OASS one trimer of the SAT subunits formed a complex with one dimer of OASS subunits .
	manualset3
131245	2	406534	5	NULL	NULL	0	NULL	0 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	SAT was reversibly inactivated on cooling to 0 degrees C. Ultracentrifugal analysis showed that SAT ( a hexamer ) was dissociated mostly into two trimers on cooling to 0 degrees C in the absence of OASS , while in the presence of OASS one trimer of the SAT subunits formed a complex with one dimer of OASS subunits .
	manualset3
131246	3	406534	5	NULL	NULL	0	NULL	Ultracentrifugal analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	SAT was reversibly inactivated on cooling to 0 degrees C. Ultracentrifugal analysis showed that SAT ( a hexamer ) was dissociated mostly into two trimers on cooling to 0 degrees C in the absence of OASS , while in the presence of OASS one trimer of the SAT subunits formed a complex with one dimer of OASS subunits .
	manualset3
131247	4	406534	5	NULL	NULL	0	NULL	SAT ( a hexamer ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	SAT was reversibly inactivated on cooling to 0 degrees C. Ultracentrifugal analysis showed that SAT ( a hexamer ) was dissociated mostly into two trimers on cooling to 0 degrees C in the absence of OASS , while in the presence of OASS one trimer of the SAT subunits formed a complex with one dimer of OASS subunits .
	manualset3
131248	5	406534	5	NULL	NULL	0	NULL	two trimers	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	SAT was reversibly inactivated on cooling to 0 degrees C. Ultracentrifugal analysis showed that SAT ( a hexamer ) was dissociated mostly into two trimers on cooling to 0 degrees C in the absence of OASS , while in the presence of OASS one trimer of the SAT subunits formed a complex with one dimer of OASS subunits .
	manualset3
131249	6	406534	5	NULL	NULL	0	NULL	0 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	SAT was reversibly inactivated on cooling to 0 degrees C. Ultracentrifugal analysis showed that SAT ( a hexamer ) was dissociated mostly into two trimers on cooling to 0 degrees C in the absence of OASS , while in the presence of OASS one trimer of the SAT subunits formed a complex with one dimer of OASS subunits .
	manualset3
131250	7	406534	5	NULL	NULL	0	NULL	absence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	SAT was reversibly inactivated on cooling to 0 degrees C. Ultracentrifugal analysis showed that SAT ( a hexamer ) was dissociated mostly into two trimers on cooling to 0 degrees C in the absence of OASS , while in the presence of OASS one trimer of the SAT subunits formed a complex with one dimer of OASS subunits .
	manualset3
131251	8	406534	5	NULL	NULL	0	NULL	OASS 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	SAT was reversibly inactivated on cooling to 0 degrees C. Ultracentrifugal analysis showed that SAT ( a hexamer ) was dissociated mostly into two trimers on cooling to 0 degrees C in the absence of OASS , while in the presence of OASS one trimer of the SAT subunits formed a complex with one dimer of OASS subunits .
	manualset3
131252	9	406534	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	SAT was reversibly inactivated on cooling to 0 degrees C. Ultracentrifugal analysis showed that SAT ( a hexamer ) was dissociated mostly into two trimers on cooling to 0 degrees C in the absence of OASS , while in the presence of OASS one trimer of the SAT subunits formed a complex with one dimer of OASS subunits .
	manualset3
131253	10	406534	5	NULL	NULL	0	NULL	OASS 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	SAT was reversibly inactivated on cooling to 0 degrees C. Ultracentrifugal analysis showed that SAT ( a hexamer ) was dissociated mostly into two trimers on cooling to 0 degrees C in the absence of OASS , while in the presence of OASS one trimer of the SAT subunits formed a complex with one dimer of OASS subunits .
	manualset3
131254	11	406534	5	NULL	NULL	0	NULL	one trimer	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	SAT was reversibly inactivated on cooling to 0 degrees C. Ultracentrifugal analysis showed that SAT ( a hexamer ) was dissociated mostly into two trimers on cooling to 0 degrees C in the absence of OASS , while in the presence of OASS one trimer of the SAT subunits formed a complex with one dimer of OASS subunits .
	manualset3
131255	12	406534	5	NULL	NULL	0	NULL	SAT subunits	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	SAT was reversibly inactivated on cooling to 0 degrees C. Ultracentrifugal analysis showed that SAT ( a hexamer ) was dissociated mostly into two trimers on cooling to 0 degrees C in the absence of OASS , while in the presence of OASS one trimer of the SAT subunits formed a complex with one dimer of OASS subunits .
	manualset3
131256	13	406534	5	NULL	NULL	0	NULL	complex 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	SAT was reversibly inactivated on cooling to 0 degrees C. Ultracentrifugal analysis showed that SAT ( a hexamer ) was dissociated mostly into two trimers on cooling to 0 degrees C in the absence of OASS , while in the presence of OASS one trimer of the SAT subunits formed a complex with one dimer of OASS subunits .
	manualset3
131257	14	406534	5	NULL	NULL	0	NULL	one dimer	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	SAT was reversibly inactivated on cooling to 0 degrees C. Ultracentrifugal analysis showed that SAT ( a hexamer ) was dissociated mostly into two trimers on cooling to 0 degrees C in the absence of OASS , while in the presence of OASS one trimer of the SAT subunits formed a complex with one dimer of OASS subunits .
	manualset3
131258	1	406535	5	NULL	NULL	0	NULL	SB204741 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	SB204741 reduced microvessel density in tumors and inhibited the proliferation of HUVEC in vitro .
	manualset3
131259	2	406535	5	NULL	NULL	0	NULL	microvessel density	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	SB204741 reduced microvessel density in tumors and inhibited the proliferation of HUVEC in vitro .
	manualset3
131260	3	406535	5	NULL	NULL	0	NULL	tumors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	SB204741 reduced microvessel density in tumors and inhibited the proliferation of HUVEC in vitro .
	manualset3
131261	4	406535	5	NULL	NULL	0	NULL	proliferation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SB204741 reduced microvessel density in tumors and inhibited the proliferation of HUVEC in vitro .
	manualset3
131262	5	406535	5	NULL	NULL	0	NULL	HUVEC 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	SB204741 reduced microvessel density in tumors and inhibited the proliferation of HUVEC in vitro .
	manualset3
131263	1	406536	5	NULL	NULL	0	NULL	SBC 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	SBC originates at Washoe Lake , NV , where there were approximately six mills that used mercury for gold and silver amalgamation in the late 1800s .
	manualset3
131264	2	406536	5	NULL	NULL	0	NULL	Washoe Lake , NV	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	SBC originates at Washoe Lake , NV , where there were approximately six mills that used mercury for gold and silver amalgamation in the late 1800s .
	manualset3
131265	3	406536	5	NULL	NULL	0	NULL	six mills	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	SBC originates at Washoe Lake , NV , where there were approximately six mills that used mercury for gold and silver amalgamation in the late 1800s .
	manualset3
131266	4	406536	5	NULL	NULL	0	NULL	mercury 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	SBC originates at Washoe Lake , NV , where there were approximately six mills that used mercury for gold and silver amalgamation in the late 1800s .
	manualset3
131267	5	406536	5	NULL	NULL	0	NULL	gold and silver amalgamation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	SBC originates at Washoe Lake , NV , where there were approximately six mills that used mercury for gold and silver amalgamation in the late 1800s .
	manualset3
131268	6	406536	5	NULL	NULL	0	NULL	late 1800s	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	SBC originates at Washoe Lake , NV , where there were approximately six mills that used mercury for gold and silver amalgamation in the late 1800s .
	manualset3
131269	1	406537	5	NULL	NULL	0	NULL	 beta-lactam antibiotic	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A new beta-lactam antibiotic , named thienamycin , was discovered in culture broths of Streptomyces MA4297 .
	manualset3
131270	2	406537	5	NULL	NULL	0	NULL	thienamycin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A new beta-lactam antibiotic , named thienamycin , was discovered in culture broths of Streptomyces MA4297 .
	manualset3
131271	3	406537	5	NULL	NULL	0	NULL	culture broths	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A new beta-lactam antibiotic , named thienamycin , was discovered in culture broths of Streptomyces MA4297 .
	manualset3
131272	4	406537	5	NULL	NULL	0	NULL	Streptomyces MA4297	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A new beta-lactam antibiotic , named thienamycin , was discovered in culture broths of Streptomyces MA4297 .
	manualset3
131273	1	406538	5	NULL	NULL	0	NULL	SCAR markers 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	SCAR markers and multiplex PCR-based identification of isomorphic species in the Anopheles dirus complex in Southeast Asia .
	manualset3
131274	2	406538	5	NULL	NULL	0	NULL	multiplex PCR-based identification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	SCAR markers and multiplex PCR-based identification of isomorphic species in the Anopheles dirus complex in Southeast Asia .
	manualset3
131275	3	406538	5	NULL	NULL	0	NULL	isomorphic species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	SCAR markers and multiplex PCR-based identification of isomorphic species in the Anopheles dirus complex in Southeast Asia .
	manualset3
131276	4	406538	5	NULL	NULL	0	NULL	Anopheles dirus complex	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	SCAR markers and multiplex PCR-based identification of isomorphic species in the Anopheles dirus complex in Southeast Asia .
	manualset3
131277	5	406538	5	NULL	NULL	0	NULL	Southeast Asia	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	SCAR markers and multiplex PCR-based identification of isomorphic species in the Anopheles dirus complex in Southeast Asia .
	manualset3
131278	1	406539	5	NULL	NULL	0	NULL	SCF 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	SCF also elicits cell-cell and cell-substratum adhesion , facilitates the proliferation , and sustains the survival , differentiation , and maturation , of mast cells .
	manualset3
131279	2	406539	5	NULL	NULL	0	NULL	 cell-cell adhesion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SCF also elicits cell-cell and cell-substratum adhesion , facilitates the proliferation , and sustains the survival , differentiation , and maturation , of mast cells .
	manualset3
131280	3	406539	5	NULL	NULL	0	NULL	cell-substratum adhesion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SCF also elicits cell-cell and cell-substratum adhesion , facilitates the proliferation , and sustains the survival , differentiation , and maturation , of mast cells .
	manualset3
131281	4	406539	5	NULL	NULL	0	NULL	proliferation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SCF also elicits cell-cell and cell-substratum adhesion , facilitates the proliferation , and sustains the survival , differentiation , and maturation , of mast cells .
	manualset3
131282	5	406539	5	NULL	NULL	0	NULL	survival 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SCF also elicits cell-cell and cell-substratum adhesion , facilitates the proliferation , and sustains the survival , differentiation , and maturation , of mast cells .
	manualset3
131283	6	406539	5	NULL	NULL	0	NULL	differentiation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SCF also elicits cell-cell and cell-substratum adhesion , facilitates the proliferation , and sustains the survival , differentiation , and maturation , of mast cells .
	manualset3
131284	7	406539	5	NULL	NULL	0	NULL	maturation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SCF also elicits cell-cell and cell-substratum adhesion , facilitates the proliferation , and sustains the survival , differentiation , and maturation , of mast cells .
	manualset3
131285	8	406539	5	NULL	NULL	0	NULL	mast cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	SCF also elicits cell-cell and cell-substratum adhesion , facilitates the proliferation , and sustains the survival , differentiation , and maturation , of mast cells .
	manualset3
131286	1	406540	5	NULL	NULL	0	NULL	SEA0400 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	SEA0400 is a selective inhibitor of the Na ( + ) / Ca ( 2 + ) exchanger having equal potencies to suppress both the forward and reverse mode operation of the Na ( + ) / Ca ( 2 + ) exchanger .
	manualset3
131287	2	406540	5	NULL	NULL	0	NULL	selective inhibitor	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	SEA0400 is a selective inhibitor of the Na ( + ) / Ca ( 2 + ) exchanger having equal potencies to suppress both the forward and reverse mode operation of the Na ( + ) / Ca ( 2 + ) exchanger .
	manualset3
131288	3	406540	5	NULL	NULL	0	NULL	Na ( + ) / Ca ( 2 + ) exchanger	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	SEA0400 is a selective inhibitor of the Na ( + ) / Ca ( 2 + ) exchanger having equal potencies to suppress both the forward and reverse mode operation of the Na ( + ) / Ca ( 2 + ) exchanger .
	manualset3
131289	4	406540	5	NULL	NULL	0	NULL	 equal potencies 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SEA0400 is a selective inhibitor of the Na ( + ) / Ca ( 2 + ) exchanger having equal potencies to suppress both the forward and reverse mode operation of the Na ( + ) / Ca ( 2 + ) exchanger .
	manualset3
131290	5	406540	5	NULL	NULL	0	NULL	forward and reverse mode operation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SEA0400 is a selective inhibitor of the Na ( + ) / Ca ( 2 + ) exchanger having equal potencies to suppress both the forward and reverse mode operation of the Na ( + ) / Ca ( 2 + ) exchanger .
	manualset3
131291	6	406540	5	NULL	NULL	0	NULL	Na ( + ) / Ca ( 2 + ) exchanger	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	SEA0400 is a selective inhibitor of the Na ( + ) / Ca ( 2 + ) exchanger having equal potencies to suppress both the forward and reverse mode operation of the Na ( + ) / Ca ( 2 + ) exchanger .
	manualset3
131292	1	406541	5	NULL	NULL	0	NULL	SEF 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	SEF contain secretory vesicles and abundant mitochondria .
	manualset3
131293	2	406541	5	NULL	NULL	0	NULL	secretory vesicles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	SEF contain secretory vesicles and abundant mitochondria .
	manualset3
131294	3	406541	5	NULL	NULL	0	NULL	mitochondria 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	SEF contain secretory vesicles and abundant mitochondria .
	manualset3
131295	1	406542	5	NULL	NULL	0	NULL	SEJCs 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	SEJCs were similar in amplitude and time course to EJCs evoked by low-frequency stimulation in the same attachment in all three tissues .
	manualset3
131296	2	406542	5	NULL	NULL	0	NULL	amplitude 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	SEJCs were similar in amplitude and time course to EJCs evoked by low-frequency stimulation in the same attachment in all three tissues .
	manualset3
131297	3	406542	5	NULL	NULL	0	NULL	time course	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	SEJCs were similar in amplitude and time course to EJCs evoked by low-frequency stimulation in the same attachment in all three tissues .
	manualset3
131298	4	406542	5	NULL	NULL	0	NULL	EJCs	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	SEJCs were similar in amplitude and time course to EJCs evoked by low-frequency stimulation in the same attachment in all three tissues .
	manualset3
131299	5	406542	5	NULL	NULL	0	NULL	low-frequency stimulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	SEJCs were similar in amplitude and time course to EJCs evoked by low-frequency stimulation in the same attachment in all three tissues .
	manualset3
131300	6	406542	5	NULL	NULL	0	NULL	attachment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	SEJCs were similar in amplitude and time course to EJCs evoked by low-frequency stimulation in the same attachment in all three tissues .
	manualset3
131301	7	406542	5	NULL	NULL	0	NULL	three 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	SEJCs were similar in amplitude and time course to EJCs evoked by low-frequency stimulation in the same attachment in all three tissues .
	manualset3
131302	8	406542	5	NULL	NULL	0	NULL	tissues 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	SEJCs were similar in amplitude and time course to EJCs evoked by low-frequency stimulation in the same attachment in all three tissues .
	manualset3
131303	1	406543	5	NULL	NULL	0	NULL	SEM values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	SEM values for SCOPA-PS and PDQ-39 SI were 11.84 and 6.72 , respectively .
	manualset3
131304	2	406543	5	NULL	NULL	0	NULL	 SCOPA-PS	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	SEM values for SCOPA-PS and PDQ-39 SI were 11.84 and 6.72 , respectively .
	manualset3
131305	3	406543	5	NULL	NULL	0	NULL	PDQ-39 SI	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	SEM values for SCOPA-PS and PDQ-39 SI were 11.84 and 6.72 , respectively .
	manualset3
131306	4	406543	5	NULL	NULL	0	NULL	11.84	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	SEM values for SCOPA-PS and PDQ-39 SI were 11.84 and 6.72 , respectively .
	manualset3
131307	5	406543	5	NULL	NULL	0	NULL	6.72	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	SEM values for SCOPA-PS and PDQ-39 SI were 11.84 and 6.72 , respectively .
	manualset3
131308	1	406544	5	NULL	NULL	NULL	NULL	SET-CAN 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	SET-CAN encodes an almost complete SET protein fused to the C-terminal two-thirds of CAN .
	manualset3
131309	2	406544	5	NULL	NULL	0	NULL	SET protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	SET-CAN encodes an almost complete SET protein fused to the C-terminal two-thirds of CAN .
	manualset3
131310	3	406544	5	NULL	NULL	0	NULL	C-terminal 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	SET-CAN encodes an almost complete SET protein fused to the C-terminal two-thirds of CAN .
	manualset3
131311	4	406544	5	NULL	NULL	0	NULL	CAN	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	SET-CAN encodes an almost complete SET protein fused to the C-terminal two-thirds of CAN .
	manualset3
131312	1	406545	5	NULL	NULL	0	NULL	SF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	SF is a glycoprotein , but glycosylation is not necessary for its activity .
	manualset3
131313	2	406545	5	NULL	NULL	0	NULL	glycoprotein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	SF is a glycoprotein , but glycosylation is not necessary for its activity .
	manualset3
131314	3	406545	5	NULL	NULL	0	NULL	glycosylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SF is a glycoprotein , but glycosylation is not necessary for its activity .
	manualset3
131315	4	406545	5	NULL	NULL	0	NULL	activity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SF is a glycoprotein , but glycosylation is not necessary for its activity .
	manualset3
131316	1	406546	5	NULL	NULL	0	NULL	SF3B1 mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SF3B1 mutations are associated with a favorable prognosis , whereas U2AF1 and SRSF2 mutations are predictive for shorter survival .
	manualset3
131317	2	406546	5	NULL	NULL	0	NULL	favorable prognosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	SF3B1 mutations are associated with a favorable prognosis , whereas U2AF1 and SRSF2 mutations are predictive for shorter survival .
	manualset3
131318	3	406546	5	NULL	NULL	0	NULL	U2AF1 mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SF3B1 mutations are associated with a favorable prognosis , whereas U2AF1 and SRSF2 mutations are predictive for shorter survival .
	manualset3
131319	4	406546	5	NULL	NULL	0	NULL	SRSF2 mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SF3B1 mutations are associated with a favorable prognosis , whereas U2AF1 and SRSF2 mutations are predictive for shorter survival .
	manualset3
131320	5	406546	5	NULL	NULL	0	NULL	shorter survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	SF3B1 mutations are associated with a favorable prognosis , whereas U2AF1 and SRSF2 mutations are predictive for shorter survival .
	manualset3
131321	1	406547	5	NULL	NULL	0	NULL	SFRP4 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	SFRP4 suppresses activation of Wnt7a signaling in both an autocrine and paracrine manner .
	manualset3
131322	2	406547	5	NULL	NULL	NULL	NULL	activation 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	SFRP4 suppresses activation of Wnt7a signaling in both an autocrine and paracrine manner .
	manualset3
131323	3	406547	5	NULL	NULL	0	NULL	Wnt7a signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SFRP4 suppresses activation of Wnt7a signaling in both an autocrine and paracrine manner .
	manualset3
131324	4	406547	5	NULL	NULL	0	NULL	autocrine manner	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SFRP4 suppresses activation of Wnt7a signaling in both an autocrine and paracrine manner .
	manualset3
131325	5	406547	5	NULL	NULL	0	NULL	paracrine manner	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SFRP4 suppresses activation of Wnt7a signaling in both an autocrine and paracrine manner .
	manualset3
131326	1	406548	5	NULL	NULL	0	NULL	SHP-1 , a SH2 domain-containing protein-tyrosine phosphatase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	SHP-1 , a SH2 domain-containing protein-tyrosine phosphatase , selectively binds and dephosphorylates PTEN in Src transfected cells .
	manualset3
131329	4	406548	5	NULL	NULL	0	NULL	PTEN 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	SHP-1 , a SH2 domain-containing protein-tyrosine phosphatase , selectively binds and dephosphorylates PTEN in Src transfected cells .
	manualset3
131330	5	406548	5	NULL	NULL	0	NULL	Src transfected cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	SHP-1 , a SH2 domain-containing protein-tyrosine phosphatase , selectively binds and dephosphorylates PTEN in Src transfected cells .
	manualset3
131331	1	406549	5	NULL	NULL	0	NULL	SI units	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	SI units of exposure in radiology .
	manualset3
131332	2	406549	5	NULL	NULL	NULL	NULL	exposure 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	SI units of exposure in radiology .
	manualset3
131333	3	406549	5	NULL	NULL	0	NULL	radiology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	SI units of exposure in radiology .
	manualset3
131334	1	406550	5	NULL	NULL	0	NULL	SIFT-MS analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	SIFT-MS analysis showed that methyl pentadiene , ethanol , isoprene and methanol were key biomarker volatiles produced by A. fumigatus in the presence of anti-fungal compounds .
	manualset3
131335	2	406550	5	NULL	NULL	0	NULL	methyl pentadiene	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	SIFT-MS analysis showed that methyl pentadiene , ethanol , isoprene and methanol were key biomarker volatiles produced by A. fumigatus in the presence of anti-fungal compounds .
	manualset3
131336	3	406550	5	NULL	NULL	0	NULL	ethanol 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	SIFT-MS analysis showed that methyl pentadiene , ethanol , isoprene and methanol were key biomarker volatiles produced by A. fumigatus in the presence of anti-fungal compounds .
	manualset3
131337	4	406550	5	NULL	NULL	0	NULL	isoprene 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	SIFT-MS analysis showed that methyl pentadiene , ethanol , isoprene and methanol were key biomarker volatiles produced by A. fumigatus in the presence of anti-fungal compounds .
	manualset3
131338	5	406550	5	NULL	NULL	0	NULL	methanol 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	SIFT-MS analysis showed that methyl pentadiene , ethanol , isoprene and methanol were key biomarker volatiles produced by A. fumigatus in the presence of anti-fungal compounds .
	manualset3
131339	6	406550	5	NULL	NULL	0	NULL	key biomarker volatiles	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	SIFT-MS analysis showed that methyl pentadiene , ethanol , isoprene and methanol were key biomarker volatiles produced by A. fumigatus in the presence of anti-fungal compounds .
	manualset3
131340	7	406550	5	NULL	NULL	0	NULL	A. fumigatus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	SIFT-MS analysis showed that methyl pentadiene , ethanol , isoprene and methanol were key biomarker volatiles produced by A. fumigatus in the presence of anti-fungal compounds .
	manualset3
131341	8	406550	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	SIFT-MS analysis showed that methyl pentadiene , ethanol , isoprene and methanol were key biomarker volatiles produced by A. fumigatus in the presence of anti-fungal compounds .
	manualset3
131342	9	406550	5	NULL	NULL	NULL	NULL	anti-fungal compounds	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	SIFT-MS analysis showed that methyl pentadiene , ethanol , isoprene and methanol were key biomarker volatiles produced by A. fumigatus in the presence of anti-fungal compounds .
	manualset3
131343	1	406551	5	NULL	NULL	0	NULL	SIT4 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	SIT4 encodes a type 2A-related protein phosphatase that is required in late G1 for normal G1 cyclin expression and for bud initiation .
	manualset3
131344	2	406551	5	NULL	NULL	0	NULL	 type 2A-related protein phosphatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	SIT4 encodes a type 2A-related protein phosphatase that is required in late G1 for normal G1 cyclin expression and for bud initiation .
	manualset3
131345	3	406551	5	NULL	NULL	0	NULL	late G1	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	SIT4 encodes a type 2A-related protein phosphatase that is required in late G1 for normal G1 cyclin expression and for bud initiation .
	manualset3
131346	4	406551	5	NULL	NULL	0	NULL	normal G1 cyclin expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SIT4 encodes a type 2A-related protein phosphatase that is required in late G1 for normal G1 cyclin expression and for bud initiation .
	manualset3
131347	5	406551	5	NULL	NULL	0	NULL	bud initiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SIT4 encodes a type 2A-related protein phosphatase that is required in late G1 for normal G1 cyclin expression and for bud initiation .
	manualset3
131348	1	406552	5	NULL	NULL	0	NULL	SJL strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	SJL and NIH strains were highly susceptible to infection with M. corti , larval burdens at 21 days after infection with 100 tetrathyridia being considerably higher ( greater than 1000 ) than all other strains .
	manualset3
131349	2	406552	5	NULL	NULL	0	NULL	NIH strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	SJL and NIH strains were highly susceptible to infection with M. corti , larval burdens at 21 days after infection with 100 tetrathyridia being considerably higher ( greater than 1000 ) than all other strains .
	manualset3
131350	3	406552	5	NULL	NULL	0	NULL	infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	SJL and NIH strains were highly susceptible to infection with M. corti , larval burdens at 21 days after infection with 100 tetrathyridia being considerably higher ( greater than 1000 ) than all other strains .
	manualset3
131351	4	406552	5	NULL	NULL	0	NULL	M. corti	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	SJL and NIH strains were highly susceptible to infection with M. corti , larval burdens at 21 days after infection with 100 tetrathyridia being considerably higher ( greater than 1000 ) than all other strains .
	manualset3
131352	5	406552	5	NULL	NULL	0	NULL	larval burdens	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	SJL and NIH strains were highly susceptible to infection with M. corti , larval burdens at 21 days after infection with 100 tetrathyridia being considerably higher ( greater than 1000 ) than all other strains .
	manualset3
131353	6	406552	5	NULL	NULL	0	NULL	21 days 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	SJL and NIH strains were highly susceptible to infection with M. corti , larval burdens at 21 days after infection with 100 tetrathyridia being considerably higher ( greater than 1000 ) than all other strains .
	manualset3
131354	7	406552	5	NULL	NULL	0	NULL	infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	SJL and NIH strains were highly susceptible to infection with M. corti , larval burdens at 21 days after infection with 100 tetrathyridia being considerably higher ( greater than 1000 ) than all other strains .
	manualset3
131355	8	406552	5	NULL	NULL	0	NULL	100 tetrathyridia 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	SJL and NIH strains were highly susceptible to infection with M. corti , larval burdens at 21 days after infection with 100 tetrathyridia being considerably higher ( greater than 1000 ) than all other strains .
	manualset3
131356	9	406552	5	NULL	NULL	0	NULL	greater than 1000	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	SJL and NIH strains were highly susceptible to infection with M. corti , larval burdens at 21 days after infection with 100 tetrathyridia being considerably higher ( greater than 1000 ) than all other strains .
	manualset3
131357	10	406552	5	NULL	NULL	0	NULL	strains 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	SJL and NIH strains were highly susceptible to infection with M. corti , larval burdens at 21 days after infection with 100 tetrathyridia being considerably higher ( greater than 1000 ) than all other strains .
	manualset3
131358	1	406553	5	NULL	NULL	0	NULL	SK3 immunoreactivity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SK3 immunoreactivity was detected in the ONL of the olfactory bulb , neural cell body and fibers of the substantia nigra and hypothalamus .
	manualset3
131359	2	406553	5	NULL	NULL	0	NULL	ONL 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	SK3 immunoreactivity was detected in the ONL of the olfactory bulb , neural cell body and fibers of the substantia nigra and hypothalamus .
	manualset3
131360	3	406553	5	NULL	NULL	0	NULL	olfactory bulb	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	SK3 immunoreactivity was detected in the ONL of the olfactory bulb , neural cell body and fibers of the substantia nigra and hypothalamus .
	manualset3
131361	4	406553	5	NULL	NULL	0	NULL	neural cell body	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	SK3 immunoreactivity was detected in the ONL of the olfactory bulb , neural cell body and fibers of the substantia nigra and hypothalamus .
	manualset3
131362	5	406553	5	NULL	NULL	0	NULL	fibers 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	SK3 immunoreactivity was detected in the ONL of the olfactory bulb , neural cell body and fibers of the substantia nigra and hypothalamus .
	manualset3
131363	6	406553	5	NULL	NULL	0	NULL	substantia nigra	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	SK3 immunoreactivity was detected in the ONL of the olfactory bulb , neural cell body and fibers of the substantia nigra and hypothalamus .
	manualset3
131364	7	406553	5	NULL	NULL	0	NULL	hypothalamus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	SK3 immunoreactivity was detected in the ONL of the olfactory bulb , neural cell body and fibers of the substantia nigra and hypothalamus .
	manualset3
131365	1	406554	5	NULL	NULL	0	NULL	chlorinated isoflavone , 3 ' , 8 - dichlorogenistein 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A new chlorinated isoflavone , 3 ' , 8 - dichlorogenistein ( 1 ) , along with 8-chlorogenistein ( 2 ) were isolated from the fermentation broth of Actinoplanes sp .
	manualset3
131366	2	406554	5	NULL	NULL	0	NULL	8-chlorogenistein	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A new chlorinated isoflavone , 3 ' , 8 - dichlorogenistein ( 1 ) , along with 8-chlorogenistein ( 2 ) were isolated from the fermentation broth of Actinoplanes sp .
	manualset3
131367	3	406554	5	NULL	NULL	0	NULL	fermentation broth	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A new chlorinated isoflavone , 3 ' , 8 - dichlorogenistein ( 1 ) , along with 8-chlorogenistein ( 2 ) were isolated from the fermentation broth of Actinoplanes sp .
	manualset3
131368	4	406554	5	NULL	NULL	0	NULL	Actinoplanes sp	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A new chlorinated isoflavone , 3 ' , 8 - dichlorogenistein ( 1 ) , along with 8-chlorogenistein ( 2 ) were isolated from the fermentation broth of Actinoplanes sp .
	manualset3
131369	1	406555	5	NULL	NULL	0	NULL	SLIR 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	SLIR was restricted to large dense-cored vesicles in processes of Ab amacrine cells .
	manualset3
131370	2	406555	5	NULL	NULL	0	NULL	large dense-cored vesicles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	SLIR was restricted to large dense-cored vesicles in processes of Ab amacrine cells .
	manualset3
131371	3	406555	5	NULL	NULL	0	NULL	processes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	SLIR was restricted to large dense-cored vesicles in processes of Ab amacrine cells .
	manualset3
131372	4	406555	5	NULL	NULL	0	NULL	Ab amacrine cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	SLIR was restricted to large dense-cored vesicles in processes of Ab amacrine cells .
	manualset3
131373	1	406556	5	NULL	NULL	0	NULL	SM-368229 , a novel selective and potent non-steroidal mineralocorticoid receptor antagonist	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	SM-368229 , a novel selective and potent non-steroidal mineralocorticoid receptor antagonist with strong urinary Na + excretion activity .
	manualset3
131374	2	406556	5	NULL	NULL	0	NULL	urinary Na + excretion activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SM-368229 , a novel selective and potent non-steroidal mineralocorticoid receptor antagonist with strong urinary Na + excretion activity .
	manualset3
131375	1	406557	5	NULL	NULL	0	NULL	SMART 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	SMART also provides a standardized format to allow dissemination of single molecule data and transparency in the analysis of reported data .
	manualset3
131376	2	406557	5	NULL	NULL	0	NULL	standardized format	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	SMART also provides a standardized format to allow dissemination of single molecule data and transparency in the analysis of reported data .
	manualset3
131377	3	406557	5	NULL	NULL	0	NULL	dissemination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	SMART also provides a standardized format to allow dissemination of single molecule data and transparency in the analysis of reported data .
	manualset3
131378	4	406557	5	NULL	NULL	0	NULL	single molecule data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	SMART also provides a standardized format to allow dissemination of single molecule data and transparency in the analysis of reported data .
	manualset3
131379	5	406557	5	NULL	NULL	0	NULL	transparency 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	SMART also provides a standardized format to allow dissemination of single molecule data and transparency in the analysis of reported data .
	manualset3
131380	6	406557	5	NULL	NULL	0	NULL	analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	SMART also provides a standardized format to allow dissemination of single molecule data and transparency in the analysis of reported data .
	manualset3
131381	7	406557	5	NULL	NULL	0	NULL	reported data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	SMART also provides a standardized format to allow dissemination of single molecule data and transparency in the analysis of reported data .
	manualset3
131382	1	406558	5	NULL	NULL	NULL	NULL	SNPs	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	SNPs in the CpG island of NAP1L2 : a possible link between DNA methylation and neural tube defects ?
	manualset3
131383	2	406558	5	NULL	NULL	0	NULL	CpG island	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	SNPs in the CpG island of NAP1L2 : a possible link between DNA methylation and neural tube defects ?
	manualset3
131384	3	406558	5	NULL	NULL	0	NULL	NAP1L2	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	SNPs in the CpG island of NAP1L2 : a possible link between DNA methylation and neural tube defects ?
	manualset3
131385	4	406558	5	NULL	NULL	0	NULL	possible link	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	SNPs in the CpG island of NAP1L2 : a possible link between DNA methylation and neural tube defects ?
	manualset3
131386	5	406558	5	NULL	NULL	0	NULL	DNA methylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SNPs in the CpG island of NAP1L2 : a possible link between DNA methylation and neural tube defects ?
	manualset3
131387	6	406558	5	NULL	NULL	0	NULL	neural tube defects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	SNPs in the CpG island of NAP1L2 : a possible link between DNA methylation and neural tube defects ?
	manualset3
131388	1	406559	5	NULL	NULL	0	NULL	SO attending	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SO attending is the behavior required to concentrate on current sensory input , whereas SI attending is the mental processing that accompanies self-generated or self-maintained thought .
	manualset3
131389	2	406559	5	NULL	NULL	0	NULL	behavior 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	SO attending is the behavior required to concentrate on current sensory input , whereas SI attending is the mental processing that accompanies self-generated or self-maintained thought .
	manualset3
131390	3	406559	5	NULL	NULL	0	NULL	concentrate 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SO attending is the behavior required to concentrate on current sensory input , whereas SI attending is the mental processing that accompanies self-generated or self-maintained thought .
	manualset3
131391	4	406559	5	NULL	NULL	0	NULL	current sensory input	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	SO attending is the behavior required to concentrate on current sensory input , whereas SI attending is the mental processing that accompanies self-generated or self-maintained thought .
	manualset3
131392	5	406559	5	NULL	NULL	0	NULL	SI attending	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SO attending is the behavior required to concentrate on current sensory input , whereas SI attending is the mental processing that accompanies self-generated or self-maintained thought .
	manualset3
131393	6	406559	5	NULL	NULL	0	NULL	mental processing	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SO attending is the behavior required to concentrate on current sensory input , whereas SI attending is the mental processing that accompanies self-generated or self-maintained thought .
	manualset3
131394	7	406559	5	NULL	NULL	0	NULL	 self-generated or self-maintained thought 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SO attending is the behavior required to concentrate on current sensory input , whereas SI attending is the mental processing that accompanies self-generated or self-maintained thought .
	manualset3
131395	1	406560	5	NULL	NULL	0	NULL	SOC 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	SOC was unrelated to intimate partner violence experiences , but an earlier stage was associated with ethnicity , economic and emotional dependence , preoccupied attachment , satisfaction with social supports , and women 's use of aggression .
	manualset3
131396	2	406560	5	NULL	NULL	0	NULL	intimate partner violence experiences	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	SOC was unrelated to intimate partner violence experiences , but an earlier stage was associated with ethnicity , economic and emotional dependence , preoccupied attachment , satisfaction with social supports , and women 's use of aggression .
	manualset3
131397	3	406560	5	NULL	NULL	0	NULL	earlier stage 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	SOC was unrelated to intimate partner violence experiences , but an earlier stage was associated with ethnicity , economic and emotional dependence , preoccupied attachment , satisfaction with social supports , and women 's use of aggression .
	manualset3
131398	4	406560	5	NULL	NULL	0	NULL	ethnicity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	SOC was unrelated to intimate partner violence experiences , but an earlier stage was associated with ethnicity , economic and emotional dependence , preoccupied attachment , satisfaction with social supports , and women 's use of aggression .
	manualset3
131399	5	406560	5	NULL	NULL	0	NULL	economic dependence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	SOC was unrelated to intimate partner violence experiences , but an earlier stage was associated with ethnicity , economic and emotional dependence , preoccupied attachment , satisfaction with social supports , and women 's use of aggression .
	manualset3
131400	6	406560	5	NULL	NULL	0	NULL	emotional dependence 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SOC was unrelated to intimate partner violence experiences , but an earlier stage was associated with ethnicity , economic and emotional dependence , preoccupied attachment , satisfaction with social supports , and women 's use of aggression .
	manualset3
131401	7	406560	5	NULL	NULL	0	NULL	preoccupied attachment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	SOC was unrelated to intimate partner violence experiences , but an earlier stage was associated with ethnicity , economic and emotional dependence , preoccupied attachment , satisfaction with social supports , and women 's use of aggression .
	manualset3
131402	8	406560	5	NULL	NULL	0	NULL	satisfaction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	SOC was unrelated to intimate partner violence experiences , but an earlier stage was associated with ethnicity , economic and emotional dependence , preoccupied attachment , satisfaction with social supports , and women 's use of aggression .
	manualset3
131403	9	406560	5	NULL	NULL	0	NULL	social supports	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	SOC was unrelated to intimate partner violence experiences , but an earlier stage was associated with ethnicity , economic and emotional dependence , preoccupied attachment , satisfaction with social supports , and women 's use of aggression .
	manualset3
131404	10	406560	5	NULL	NULL	0	NULL	women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	SOC was unrelated to intimate partner violence experiences , but an earlier stage was associated with ethnicity , economic and emotional dependence , preoccupied attachment , satisfaction with social supports , and women 's use of aggression .
	manualset3
131405	11	406560	5	NULL	NULL	0	NULL	aggression 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	SOC was unrelated to intimate partner violence experiences , but an earlier stage was associated with ethnicity , economic and emotional dependence , preoccupied attachment , satisfaction with social supports , and women 's use of aggression .
	manualset3
131406	1	406561	5	NULL	NULL	0	NULL	new class	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new class of fluorescence sensors for ammonium and organoammonium ions has been disclosed .
	manualset3
131407	2	406561	5	NULL	NULL	0	NULL	fluorescence sensors	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A new class of fluorescence sensors for ammonium and organoammonium ions has been disclosed .
	manualset3
131408	3	406561	5	NULL	NULL	0	NULL	ammonium ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	A new class of fluorescence sensors for ammonium and organoammonium ions has been disclosed .
	manualset3
131409	4	406561	5	NULL	NULL	0	NULL	organoammonium ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	A new class of fluorescence sensors for ammonium and organoammonium ions has been disclosed .
	manualset3
131410	1	406562	5	NULL	NULL	0	NULL	SOM230 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	SOM230 significantly reduced cell proliferation while the conventional analog SMS201-995 did not .
	manualset3
131411	2	406562	5	NULL	NULL	0	NULL	cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SOM230 significantly reduced cell proliferation while the conventional analog SMS201-995 did not .
	manualset3
131412	3	406562	5	NULL	NULL	0	NULL	conventional analog SMS201-995	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	SOM230 significantly reduced cell proliferation while the conventional analog SMS201-995 did not .
	manualset3
131413	1	406563	5	NULL	NULL	0	NULL	SRS ( Sequence Retrieval System )	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	SRS ( Sequence Retrieval System ) is an information indexing and retrieval system designed for libraries with a flat file format such as the EMBL nucleotide sequence databank , the SwissProt protein sequence databank or the Prosite library of protein subsequence consensus patterns .
	manualset3
131414	2	406563	5	NULL	NULL	0	NULL	information indexing and retrieval system	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	SRS ( Sequence Retrieval System ) is an information indexing and retrieval system designed for libraries with a flat file format such as the EMBL nucleotide sequence databank , the SwissProt protein sequence databank or the Prosite library of protein subsequence consensus patterns .
	manualset3
131415	3	406563	5	NULL	NULL	0	NULL	libraries 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	SRS ( Sequence Retrieval System ) is an information indexing and retrieval system designed for libraries with a flat file format such as the EMBL nucleotide sequence databank , the SwissProt protein sequence databank or the Prosite library of protein subsequence consensus patterns .
	manualset3
131416	4	406563	5	NULL	NULL	0	NULL	flat file format	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	SRS ( Sequence Retrieval System ) is an information indexing and retrieval system designed for libraries with a flat file format such as the EMBL nucleotide sequence databank , the SwissProt protein sequence databank or the Prosite library of protein subsequence consensus patterns .
	manualset3
131417	5	406563	5	NULL	NULL	0	NULL	EMBL nucleotide sequence databank	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	SRS ( Sequence Retrieval System ) is an information indexing and retrieval system designed for libraries with a flat file format such as the EMBL nucleotide sequence databank , the SwissProt protein sequence databank or the Prosite library of protein subsequence consensus patterns .
	manualset3
131418	6	406563	5	NULL	NULL	0	NULL	SwissProt protein sequence databank	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	SRS ( Sequence Retrieval System ) is an information indexing and retrieval system designed for libraries with a flat file format such as the EMBL nucleotide sequence databank , the SwissProt protein sequence databank or the Prosite library of protein subsequence consensus patterns .
	manualset3
131419	7	406563	5	NULL	NULL	0	NULL	Prosite library	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	SRS ( Sequence Retrieval System ) is an information indexing and retrieval system designed for libraries with a flat file format such as the EMBL nucleotide sequence databank , the SwissProt protein sequence databank or the Prosite library of protein subsequence consensus patterns .
	manualset3
131420	8	406563	5	NULL	NULL	0	NULL	protein subsequence consensus patterns	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	SRS ( Sequence Retrieval System ) is an information indexing and retrieval system designed for libraries with a flat file format such as the EMBL nucleotide sequence databank , the SwissProt protein sequence databank or the Prosite library of protein subsequence consensus patterns .
	manualset3
131421	1	406564	5	NULL	NULL	0	NULL	SSTR-scan	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	SSTR-scan provided information about SSTR-expression , tumor viability and extension .
	manualset3
131422	2	406564	5	NULL	NULL	0	NULL	information 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	SSTR-scan provided information about SSTR-expression , tumor viability and extension .
	manualset3
131423	3	406564	5	NULL	NULL	0	NULL	SSTR-expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SSTR-scan provided information about SSTR-expression , tumor viability and extension .
	manualset3
131424	4	406564	5	NULL	NULL	0	NULL	tumor viability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	SSTR-scan provided information about SSTR-expression , tumor viability and extension .
	manualset3
131425	5	406564	5	NULL	NULL	0	NULL	extension 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	SSTR-scan provided information about SSTR-expression , tumor viability and extension .
	manualset3
131426	1	406565	5	NULL	NULL	0	NULL	Growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	STARTING POINT : Growth and migration of vascular smooth-muscle cells result in neointimal proliferation after vascular injury and are the key mechanism of in-stent restenosis .
	manualset3
131427	2	406565	5	NULL	NULL	0	NULL	migration 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	STARTING POINT : Growth and migration of vascular smooth-muscle cells result in neointimal proliferation after vascular injury and are the key mechanism of in-stent restenosis .
	manualset3
131428	3	406565	5	NULL	NULL	0	NULL	vascular smooth-muscle cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	STARTING POINT : Growth and migration of vascular smooth-muscle cells result in neointimal proliferation after vascular injury and are the key mechanism of in-stent restenosis .
	manualset3
131429	4	406565	5	NULL	NULL	0	NULL	neointimal proliferation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	STARTING POINT : Growth and migration of vascular smooth-muscle cells result in neointimal proliferation after vascular injury and are the key mechanism of in-stent restenosis .
	manualset3
131430	5	406565	5	NULL	NULL	0	NULL	vascular injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	STARTING POINT : Growth and migration of vascular smooth-muscle cells result in neointimal proliferation after vascular injury and are the key mechanism of in-stent restenosis .
	manualset3
131431	6	406565	5	NULL	NULL	0	NULL	 key mechanism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	STARTING POINT : Growth and migration of vascular smooth-muscle cells result in neointimal proliferation after vascular injury and are the key mechanism of in-stent restenosis .
	manualset3
131432	7	406565	5	NULL	NULL	0	NULL	in-stent restenosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	STARTING POINT : Growth and migration of vascular smooth-muscle cells result in neointimal proliferation after vascular injury and are the key mechanism of in-stent restenosis .
	manualset3
131433	1	406566	5	NULL	NULL	0	NULL	STAT3 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	STAT3 and phosphorylated SMAD1/5/8 proteins were analyzed by Western blot .
	manualset3
131434	2	406566	5	NULL	NULL	0	NULL	phosphorylated SMAD1/5/8 proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	STAT3 and phosphorylated SMAD1/5/8 proteins were analyzed by Western blot .
	manualset3
131435	3	406566	5	NULL	NULL	0	NULL	Western blot	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	STAT3 and phosphorylated SMAD1/5/8 proteins were analyzed by Western blot .
	manualset3
131436	1	406567	5	NULL	NULL	0	NULL	STAT3 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	STAT3 mediates hepatic hepcidin expression and its inflammatory stimulation .
	manualset3
131437	2	406567	5	NULL	NULL	0	NULL	hepatic hepcidin expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	STAT3 mediates hepatic hepcidin expression and its inflammatory stimulation .
	manualset3
131438	3	406567	5	NULL	NULL	0	NULL	inflammatory stimulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	STAT3 mediates hepatic hepcidin expression and its inflammatory stimulation .
	manualset3
131439	1	406568	5	NULL	NULL	0	NULL	new class	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new class of phenyl ( pyridylalcyl ) guanidines , acting as potent histamine H2-agonists , inhibits IgE-mediated human basophil histamine release in a nanomolar range .
	manualset3
131440	2	406568	5	NULL	NULL	0	NULL	 phenyl ( pyridylalcyl ) guanidines	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A new class of phenyl ( pyridylalcyl ) guanidines , acting as potent histamine H2-agonists , inhibits IgE-mediated human basophil histamine release in a nanomolar range .
	manualset3
131441	3	406568	5	NULL	NULL	0	NULL	potent histamine H2-agonists	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A new class of phenyl ( pyridylalcyl ) guanidines , acting as potent histamine H2-agonists , inhibits IgE-mediated human basophil histamine release in a nanomolar range .
	manualset3
131442	4	406568	5	NULL	NULL	0	NULL	IgE-mediated human basophil histamine release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A new class of phenyl ( pyridylalcyl ) guanidines , acting as potent histamine H2-agonists , inhibits IgE-mediated human basophil histamine release in a nanomolar range .
	manualset3
131443	5	406568	5	NULL	NULL	0	NULL	nanomolar range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new class of phenyl ( pyridylalcyl ) guanidines , acting as potent histamine H2-agonists , inhibits IgE-mediated human basophil histamine release in a nanomolar range .
	manualset3
131444	1	406569	5	NULL	NULL	0	NULL	SUMMARY 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	SUMMARY OF BACKGROUND DATA. : The indications for intervention in patients with atlantoaxial instability are pain , myelopathy , and progressive neurologic deficit .
	manualset3
131445	2	406569	5	NULL	NULL	0	NULL	BACKGROUND DATA	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	SUMMARY OF BACKGROUND DATA. : The indications for intervention in patients with atlantoaxial instability are pain , myelopathy , and progressive neurologic deficit .
	manualset3
131446	3	406569	5	NULL	NULL	0	NULL	indications 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	SUMMARY OF BACKGROUND DATA. : The indications for intervention in patients with atlantoaxial instability are pain , myelopathy , and progressive neurologic deficit .
	manualset3
131447	4	406569	5	NULL	NULL	0	NULL	intervention 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	SUMMARY OF BACKGROUND DATA. : The indications for intervention in patients with atlantoaxial instability are pain , myelopathy , and progressive neurologic deficit .
	manualset3
131448	5	406569	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	SUMMARY OF BACKGROUND DATA. : The indications for intervention in patients with atlantoaxial instability are pain , myelopathy , and progressive neurologic deficit .
	manualset3
131449	6	406569	5	NULL	NULL	0	NULL	atlantoaxial instability 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	SUMMARY OF BACKGROUND DATA. : The indications for intervention in patients with atlantoaxial instability are pain , myelopathy , and progressive neurologic deficit .
	manualset3
131450	7	406569	5	NULL	NULL	0	NULL	pain 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	SUMMARY OF BACKGROUND DATA. : The indications for intervention in patients with atlantoaxial instability are pain , myelopathy , and progressive neurologic deficit .
	manualset3
131451	8	406569	5	NULL	NULL	0	NULL	myelopathy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	SUMMARY OF BACKGROUND DATA. : The indications for intervention in patients with atlantoaxial instability are pain , myelopathy , and progressive neurologic deficit .
	manualset3
131452	9	406569	5	NULL	NULL	0	NULL	progressive neurologic deficit	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	SUMMARY OF BACKGROUND DATA. : The indications for intervention in patients with atlantoaxial instability are pain , myelopathy , and progressive neurologic deficit .
	manualset3
131453	1	406570	5	NULL	NULL	0	NULL	SYSTEMIC PERSPECTIVES 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	SYSTEMIC PERSPECTIVES TO THE EVOLUTION OF THE HUMAN CRANIAL MORPHOLOGY : Concepts like morphological modularity , anatomical integration , and heterochrony represent key issues in the development of the current human evolutionary studies .
	manualset3
131454	2	406570	5	NULL	NULL	0	NULL	EVOLUTION 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SYSTEMIC PERSPECTIVES TO THE EVOLUTION OF THE HUMAN CRANIAL MORPHOLOGY : Concepts like morphological modularity , anatomical integration , and heterochrony represent key issues in the development of the current human evolutionary studies .
	manualset3
131455	3	406570	5	NULL	NULL	0	NULL	HUMAN CRANIAL MORPHOLOGY	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	SYSTEMIC PERSPECTIVES TO THE EVOLUTION OF THE HUMAN CRANIAL MORPHOLOGY : Concepts like morphological modularity , anatomical integration , and heterochrony represent key issues in the development of the current human evolutionary studies .
	manualset3
131456	4	406570	5	NULL	NULL	0	NULL	Concepts 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	SYSTEMIC PERSPECTIVES TO THE EVOLUTION OF THE HUMAN CRANIAL MORPHOLOGY : Concepts like morphological modularity , anatomical integration , and heterochrony represent key issues in the development of the current human evolutionary studies .
	manualset3
131457	5	406570	5	NULL	NULL	0	NULL	morphological modularity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	SYSTEMIC PERSPECTIVES TO THE EVOLUTION OF THE HUMAN CRANIAL MORPHOLOGY : Concepts like morphological modularity , anatomical integration , and heterochrony represent key issues in the development of the current human evolutionary studies .
	manualset3
131458	6	406570	5	NULL	NULL	0	NULL	anatomical integration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	SYSTEMIC PERSPECTIVES TO THE EVOLUTION OF THE HUMAN CRANIAL MORPHOLOGY : Concepts like morphological modularity , anatomical integration , and heterochrony represent key issues in the development of the current human evolutionary studies .
	manualset3
131459	7	406570	5	NULL	NULL	0	NULL	heterochrony 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	SYSTEMIC PERSPECTIVES TO THE EVOLUTION OF THE HUMAN CRANIAL MORPHOLOGY : Concepts like morphological modularity , anatomical integration , and heterochrony represent key issues in the development of the current human evolutionary studies .
	manualset3
131460	8	406570	5	NULL	NULL	0	NULL	key issues	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	SYSTEMIC PERSPECTIVES TO THE EVOLUTION OF THE HUMAN CRANIAL MORPHOLOGY : Concepts like morphological modularity , anatomical integration , and heterochrony represent key issues in the development of the current human evolutionary studies .
	manualset3
131461	9	406570	5	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SYSTEMIC PERSPECTIVES TO THE EVOLUTION OF THE HUMAN CRANIAL MORPHOLOGY : Concepts like morphological modularity , anatomical integration , and heterochrony represent key issues in the development of the current human evolutionary studies .
	manualset3
131462	10	406570	5	NULL	NULL	0	NULL	current human evolutionary studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	SYSTEMIC PERSPECTIVES TO THE EVOLUTION OF THE HUMAN CRANIAL MORPHOLOGY : Concepts like morphological modularity , anatomical integration , and heterochrony represent key issues in the development of the current human evolutionary studies .
	manualset3
131463	1	406571	5	NULL	NULL	0	NULL	Sabi virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sabi virus , one of five arenaviruses from South America known to cause hemorrhagic fever in humans , emerged in 1990 when it was isolated from a fatal case in Sao Paulo , Brazil .
	manualset3
131464	2	406571	5	NULL	NULL	0	NULL	one of five	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sabi virus , one of five arenaviruses from South America known to cause hemorrhagic fever in humans , emerged in 1990 when it was isolated from a fatal case in Sao Paulo , Brazil .
	manualset3
131465	3	406571	5	NULL	NULL	0	NULL	arenaviruses 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sabi virus , one of five arenaviruses from South America known to cause hemorrhagic fever in humans , emerged in 1990 when it was isolated from a fatal case in Sao Paulo , Brazil .
	manualset3
131466	4	406571	5	NULL	NULL	0	NULL	South America	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Sabi virus , one of five arenaviruses from South America known to cause hemorrhagic fever in humans , emerged in 1990 when it was isolated from a fatal case in Sao Paulo , Brazil .
	manualset3
131467	5	406571	5	NULL	NULL	0	NULL	hemorrhagic fever	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Sabi virus , one of five arenaviruses from South America known to cause hemorrhagic fever in humans , emerged in 1990 when it was isolated from a fatal case in Sao Paulo , Brazil .
	manualset3
131468	6	406571	5	NULL	NULL	0	NULL	humans 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sabi virus , one of five arenaviruses from South America known to cause hemorrhagic fever in humans , emerged in 1990 when it was isolated from a fatal case in Sao Paulo , Brazil .
	manualset3
131469	7	406571	5	NULL	NULL	0	NULL	1990 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Sabi virus , one of five arenaviruses from South America known to cause hemorrhagic fever in humans , emerged in 1990 when it was isolated from a fatal case in Sao Paulo , Brazil .
	manualset3
131470	8	406571	5	NULL	NULL	0	NULL	fatal case	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Sabi virus , one of five arenaviruses from South America known to cause hemorrhagic fever in humans , emerged in 1990 when it was isolated from a fatal case in Sao Paulo , Brazil .
	manualset3
131471	9	406571	5	NULL	NULL	0	NULL	Sao Paulo , Brazil	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Sabi virus , one of five arenaviruses from South America known to cause hemorrhagic fever in humans , emerged in 1990 when it was isolated from a fatal case in Sao Paulo , Brazil .
	manualset3
131472	1	406572	5	NULL	NULL	0	NULL	new coating	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new coating for cheese , to be introduced in May , consists entirely of natural degradable components .
	manualset3
131473	2	406572	5	NULL	NULL	0	NULL	cheese 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A new coating for cheese , to be introduced in May , consists entirely of natural degradable components .
	manualset3
131474	3	406572	5	NULL	NULL	0	NULL	May 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	A new coating for cheese , to be introduced in May , consists entirely of natural degradable components .
	manualset3
131475	4	406572	5	NULL	NULL	0	NULL	natural degradable components	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A new coating for cheese , to be introduced in May , consists entirely of natural degradable components .
	manualset3
131476	1	406573	5	NULL	NULL	0	NULL	Saccharomyces cerevisiae Nfs1p	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Saccharomyces cerevisiae Nfs1p is mainly found in the mitochondrial matrix and has been shown to participate in iron-sulfur cluster assembly .
	manualset3
131477	2	406573	5	NULL	NULL	0	NULL	mitochondrial matrix	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Saccharomyces cerevisiae Nfs1p is mainly found in the mitochondrial matrix and has been shown to participate in iron-sulfur cluster assembly .
	manualset3
131478	3	406573	5	NULL	NULL	0	NULL	iron-sulfur cluster assembly	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Saccharomyces cerevisiae Nfs1p is mainly found in the mitochondrial matrix and has been shown to participate in iron-sulfur cluster assembly .
	manualset3
131479	1	406574	5	NULL	NULL	0	NULL	adolescent breast	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Sacrifice of the adolescent breast at the initial procedure is strongly discouraged .
	manualset3
131480	2	406574	5	NULL	NULL	0	NULL	initial procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Sacrifice of the adolescent breast at the initial procedure is strongly discouraged .
	manualset3
131481	1	406575	5	NULL	NULL	0	NULL	Safety 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety , tolerability , and antibody response of active A immunotherapy with CAD106 in patients with Alzheimer 's disease : randomised , double-blind , placebo-controlled , first-in-human study .
	manualset3
131482	2	406575	5	NULL	NULL	0	NULL	tolerability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety , tolerability , and antibody response of active A immunotherapy with CAD106 in patients with Alzheimer 's disease : randomised , double-blind , placebo-controlled , first-in-human study .
	manualset3
131483	3	406575	5	NULL	NULL	0	NULL	antibody response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety , tolerability , and antibody response of active A immunotherapy with CAD106 in patients with Alzheimer 's disease : randomised , double-blind , placebo-controlled , first-in-human study .
	manualset3
131484	4	406575	5	NULL	NULL	0	NULL	active A immunotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety , tolerability , and antibody response of active A immunotherapy with CAD106 in patients with Alzheimer 's disease : randomised , double-blind , placebo-controlled , first-in-human study .
	manualset3
131485	5	406575	5	NULL	NULL	0	NULL	CAD106 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety , tolerability , and antibody response of active A immunotherapy with CAD106 in patients with Alzheimer 's disease : randomised , double-blind , placebo-controlled , first-in-human study .
	manualset3
131486	6	406575	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety , tolerability , and antibody response of active A immunotherapy with CAD106 in patients with Alzheimer 's disease : randomised , double-blind , placebo-controlled , first-in-human study .
	manualset3
131487	7	406575	5	NULL	NULL	0	NULL	Alzheimer 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety , tolerability , and antibody response of active A immunotherapy with CAD106 in patients with Alzheimer 's disease : randomised , double-blind , placebo-controlled , first-in-human study .
	manualset3
131488	8	406575	5	NULL	NULL	0	NULL	randomised , double-blind , placebo-controlled , first-in-human study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety , tolerability , and antibody response of active A immunotherapy with CAD106 in patients with Alzheimer 's disease : randomised , double-blind , placebo-controlled , first-in-human study .
	manualset3
131489	1	406576	5	NULL	NULL	0	NULL	Safety 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety and efficacy of stereotactic radiosurgery for tumors of the spine .
	manualset3
131490	2	406576	5	NULL	NULL	0	NULL	efficacy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety and efficacy of stereotactic radiosurgery for tumors of the spine .
	manualset3
131491	3	406576	5	NULL	NULL	0	NULL	stereotactic radiosurgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety and efficacy of stereotactic radiosurgery for tumors of the spine .
	manualset3
131492	4	406576	5	NULL	NULL	0	NULL	tumors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety and efficacy of stereotactic radiosurgery for tumors of the spine .
	manualset3
131493	5	406576	5	NULL	NULL	0	NULL	spine 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety and efficacy of stereotactic radiosurgery for tumors of the spine .
	manualset3
131494	1	406577	5	NULL	NULL	0	NULL	Safety 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety and efficacy of warfarin in paediatric patients with prosthetic cardiac valves : a retrospective audit .
	manualset3
131495	2	406577	5	NULL	NULL	0	NULL	efficacy 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety and efficacy of warfarin in paediatric patients with prosthetic cardiac valves : a retrospective audit .
	manualset3
131496	3	406577	5	NULL	NULL	0	NULL	warfarin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety and efficacy of warfarin in paediatric patients with prosthetic cardiac valves : a retrospective audit .
	manualset3
131497	4	406577	5	NULL	NULL	0	NULL	paediatric patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety and efficacy of warfarin in paediatric patients with prosthetic cardiac valves : a retrospective audit .
	manualset3
131498	5	406577	5	NULL	NULL	0	NULL	prosthetic cardiac valves	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety and efficacy of warfarin in paediatric patients with prosthetic cardiac valves : a retrospective audit .
	manualset3
131499	6	406577	5	NULL	NULL	0	NULL	retrospective audit 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety and efficacy of warfarin in paediatric patients with prosthetic cardiac valves : a retrospective audit .
	manualset3
131500	1	406578	5	NULL	NULL	0	NULL	Safety 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety and efficacy of xenon in routine use as an inhalational anesthetic .
	manualset3
131501	2	406578	5	NULL	NULL	0	NULL	efficacy 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety and efficacy of xenon in routine use as an inhalational anesthetic .
	manualset3
131502	3	406578	5	NULL	NULL	0	NULL	xenon 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety and efficacy of xenon in routine use as an inhalational anesthetic .
	manualset3
131503	4	406578	5	NULL	NULL	0	NULL	inhalational anesthetic	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety and efficacy of xenon in routine use as an inhalational anesthetic .
	manualset3
131504	1	406579	5	NULL	NULL	0	NULL	Safety 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety of Mycoplasma gallisepticum vaccine strain 6/85 after backpassage in turkeys .
	manualset3
131505	2	406579	5	NULL	NULL	0	NULL	Mycoplasma gallisepticum vaccine strain 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety of Mycoplasma gallisepticum vaccine strain 6/85 after backpassage in turkeys .
	manualset3
131506	3	406579	5	NULL	NULL	0	NULL	6/85 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety of Mycoplasma gallisepticum vaccine strain 6/85 after backpassage in turkeys .
	manualset3
131507	4	406579	5	NULL	NULL	0	NULL	backpassage 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety of Mycoplasma gallisepticum vaccine strain 6/85 after backpassage in turkeys .
	manualset3
131508	5	406579	5	NULL	NULL	0	NULL	turkeys 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety of Mycoplasma gallisepticum vaccine strain 6/85 after backpassage in turkeys .
	manualset3
131509	1	406580	5	NULL	NULL	0	NULL	Safety 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety of antiepileptic drugs during pregnancy .
	manualset3
131510	2	406580	5	NULL	NULL	0	NULL	antiepileptic drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety of antiepileptic drugs during pregnancy .
	manualset3
131511	3	406580	5	NULL	NULL	0	NULL	pregnancy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety of antiepileptic drugs during pregnancy .
	manualset3
131512	1	406581	5	NULL	NULL	0	NULL	Safety 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety of deferasirox in sickle cell disease patients with co-existing liver impairment .
	manualset3
131513	2	406581	5	NULL	NULL	0	NULL	deferasirox 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety of deferasirox in sickle cell disease patients with co-existing liver impairment .
	manualset3
131514	3	406581	5	NULL	NULL	0	NULL	sickle cell disease patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety of deferasirox in sickle cell disease patients with co-existing liver impairment .
	manualset3
131515	4	406581	5	NULL	NULL	0	NULL	co-existing liver impairment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety of deferasirox in sickle cell disease patients with co-existing liver impairment .
	manualset3
131516	1	406582	5	NULL	NULL	0	NULL	Sagittal T2 weighted image	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Sagittal T2 weighted image of case 1 showed multiple small lesions along with the pericallosal branches from the truncus to the posterior part of the splenium in the corpus callosum .
	manualset3
131517	2	406582	5	NULL	NULL	0	NULL	 case 1	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sagittal T2 weighted image of case 1 showed multiple small lesions along with the pericallosal branches from the truncus to the posterior part of the splenium in the corpus callosum .
	manualset3
131518	3	406582	5	NULL	NULL	0	NULL	multiple small lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sagittal T2 weighted image of case 1 showed multiple small lesions along with the pericallosal branches from the truncus to the posterior part of the splenium in the corpus callosum .
	manualset3
131519	4	406582	5	NULL	NULL	0	NULL	pericallosal branches 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Sagittal T2 weighted image of case 1 showed multiple small lesions along with the pericallosal branches from the truncus to the posterior part of the splenium in the corpus callosum .
	manualset3
131520	5	406582	5	NULL	NULL	0	NULL	truncus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Sagittal T2 weighted image of case 1 showed multiple small lesions along with the pericallosal branches from the truncus to the posterior part of the splenium in the corpus callosum .
	manualset3
131521	6	406582	5	NULL	NULL	0	NULL	posterior part of the splenium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Sagittal T2 weighted image of case 1 showed multiple small lesions along with the pericallosal branches from the truncus to the posterior part of the splenium in the corpus callosum .
	manualset3
131522	7	406582	5	NULL	NULL	0	NULL	corpus callosum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Sagittal T2 weighted image of case 1 showed multiple small lesions along with the pericallosal branches from the truncus to the posterior part of the splenium in the corpus callosum .
	manualset3
131523	1	406583	5	NULL	NULL	0	NULL	Sagittal section	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sagittal section of pelvis was studied .
	manualset3
131524	2	406583	5	NULL	NULL	0	NULL	pelvis 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Sagittal section of pelvis was studied .
	manualset3
131525	1	406584	5	NULL	NULL	0	NULL	Sagittal sinus thrombosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sagittal sinus thrombosis associated with thrombocytopenia : a report of two patients .
	manualset3
131526	2	406584	5	NULL	NULL	0	NULL	thrombocytopenia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sagittal sinus thrombosis associated with thrombocytopenia : a report of two patients .
	manualset3
131527	3	406584	5	NULL	NULL	0	NULL	report 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Sagittal sinus thrombosis associated with thrombocytopenia : a report of two patients .
	manualset3
131528	4	406584	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sagittal sinus thrombosis associated with thrombocytopenia : a report of two patients .
	manualset3
131529	5	406584	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sagittal sinus thrombosis associated with thrombocytopenia : a report of two patients .
	manualset3
131530	1	406585	5	NULL	NULL	0	NULL	Saikosaponins 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Saikosaponins are triterpene saponins derived from the roots of Bupleurum falcatum L. ( Umbelliferae ) , which has been traditionally used to treat fever , inflammation , liver diseases , and nephritis .
	manualset3
131531	2	406585	5	NULL	NULL	0	NULL	triterpene saponins	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Saikosaponins are triterpene saponins derived from the roots of Bupleurum falcatum L. ( Umbelliferae ) , which has been traditionally used to treat fever , inflammation , liver diseases , and nephritis .
	manualset3
131532	3	406585	5	NULL	NULL	0	NULL	roots 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Saikosaponins are triterpene saponins derived from the roots of Bupleurum falcatum L. ( Umbelliferae ) , which has been traditionally used to treat fever , inflammation , liver diseases , and nephritis .
	manualset3
131533	4	406585	5	NULL	NULL	0	NULL	Bupleurum falcatum L. ( Umbelliferae )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Saikosaponins are triterpene saponins derived from the roots of Bupleurum falcatum L. ( Umbelliferae ) , which has been traditionally used to treat fever , inflammation , liver diseases , and nephritis .
	manualset3
131535	6	406585	5	NULL	NULL	NULL	NULL	fever 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Saikosaponins are triterpene saponins derived from the roots of Bupleurum falcatum L. ( Umbelliferae ) , which has been traditionally used to treat fever , inflammation , liver diseases , and nephritis .
	manualset3
131536	7	406585	5	NULL	NULL	0	NULL	inflammation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Saikosaponins are triterpene saponins derived from the roots of Bupleurum falcatum L. ( Umbelliferae ) , which has been traditionally used to treat fever , inflammation , liver diseases , and nephritis .
	manualset3
131537	8	406585	5	NULL	NULL	0	NULL	liver diseases 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Saikosaponins are triterpene saponins derived from the roots of Bupleurum falcatum L. ( Umbelliferae ) , which has been traditionally used to treat fever , inflammation , liver diseases , and nephritis .
	manualset3
131538	9	406585	5	NULL	NULL	0	NULL	nephritis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Saikosaponins are triterpene saponins derived from the roots of Bupleurum falcatum L. ( Umbelliferae ) , which has been traditionally used to treat fever , inflammation , liver diseases , and nephritis .
	manualset3
131539	1	406586	5	NULL	NULL	NULL	NULL	Salacinol , a naturally occurring alpha-glucosidase inhibitor	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Salacinol , a naturally occurring alpha-glucosidase inhibitor , was shown to be one of the active principles of the aqueous extract of a medicinal plant that has been prescribed traditionally as an Ayurvedic treatment for type II diabetes .
	manualset3
131540	2	406586	5	NULL	NULL	0	NULL	one 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Salacinol , a naturally occurring alpha-glucosidase inhibitor , was shown to be one of the active principles of the aqueous extract of a medicinal plant that has been prescribed traditionally as an Ayurvedic treatment for type II diabetes .
	manualset3
131541	3	406586	5	NULL	NULL	0	NULL	active principles	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Salacinol , a naturally occurring alpha-glucosidase inhibitor , was shown to be one of the active principles of the aqueous extract of a medicinal plant that has been prescribed traditionally as an Ayurvedic treatment for type II diabetes .
	manualset3
131542	4	406586	5	NULL	NULL	0	NULL	aqueous extract	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Salacinol , a naturally occurring alpha-glucosidase inhibitor , was shown to be one of the active principles of the aqueous extract of a medicinal plant that has been prescribed traditionally as an Ayurvedic treatment for type II diabetes .
	manualset3
131543	5	406586	5	NULL	NULL	0	NULL	medicinal plant	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Salacinol , a naturally occurring alpha-glucosidase inhibitor , was shown to be one of the active principles of the aqueous extract of a medicinal plant that has been prescribed traditionally as an Ayurvedic treatment for type II diabetes .
	manualset3
131544	6	406586	5	NULL	NULL	0	NULL	Ayurvedic treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Salacinol , a naturally occurring alpha-glucosidase inhibitor , was shown to be one of the active principles of the aqueous extract of a medicinal plant that has been prescribed traditionally as an Ayurvedic treatment for type II diabetes .
	manualset3
131545	7	406586	5	NULL	NULL	0	NULL	type II diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Salacinol , a naturally occurring alpha-glucosidase inhibitor , was shown to be one of the active principles of the aqueous extract of a medicinal plant that has been prescribed traditionally as an Ayurvedic treatment for type II diabetes .
	manualset3
131546	1	406587	5	NULL	NULL	0	NULL	Salen-manganese complexes	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Salen-manganese complexes exhibit powerful superoxide dismutase and catalase activity , with pharmacologic efficacy in several oxidative-stress-associated disease models .
	manualset3
131547	2	406587	5	NULL	NULL	0	NULL	superoxide dismutase activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Salen-manganese complexes exhibit powerful superoxide dismutase and catalase activity , with pharmacologic efficacy in several oxidative-stress-associated disease models .
	manualset3
131548	3	406587	5	NULL	NULL	0	NULL	catalase activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Salen-manganese complexes exhibit powerful superoxide dismutase and catalase activity , with pharmacologic efficacy in several oxidative-stress-associated disease models .
	manualset3
131549	4	406587	5	NULL	NULL	0	NULL	pharmacologic efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Salen-manganese complexes exhibit powerful superoxide dismutase and catalase activity , with pharmacologic efficacy in several oxidative-stress-associated disease models .
	manualset3
131550	5	406587	5	NULL	NULL	0	NULL	oxidative-stress-associated disease models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Salen-manganese complexes exhibit powerful superoxide dismutase and catalase activity , with pharmacologic efficacy in several oxidative-stress-associated disease models .
	manualset3
131551	1	406588	5	NULL	NULL	0	NULL	Salicylic acid deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Salicylic acid deficiency also improved seed composition in terms of antioxidant vitamin concentrations , seeds of salicylic acid-deficient plants showing higher levels of alpha - and gamma-tocopherol ( vitamin E ) and beta-carotene ( pro-vitamin A ) than seeds of wild-type plants .
	manualset3
131552	2	406588	5	NULL	NULL	0	NULL	seed composition	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Salicylic acid deficiency also improved seed composition in terms of antioxidant vitamin concentrations , seeds of salicylic acid-deficient plants showing higher levels of alpha - and gamma-tocopherol ( vitamin E ) and beta-carotene ( pro-vitamin A ) than seeds of wild-type plants .
	manualset3
131553	3	406588	5	NULL	NULL	0	NULL	antioxidant vitamin concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Salicylic acid deficiency also improved seed composition in terms of antioxidant vitamin concentrations , seeds of salicylic acid-deficient plants showing higher levels of alpha - and gamma-tocopherol ( vitamin E ) and beta-carotene ( pro-vitamin A ) than seeds of wild-type plants .
	manualset3
131554	4	406588	5	NULL	NULL	0	NULL	seeds 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Salicylic acid deficiency also improved seed composition in terms of antioxidant vitamin concentrations , seeds of salicylic acid-deficient plants showing higher levels of alpha - and gamma-tocopherol ( vitamin E ) and beta-carotene ( pro-vitamin A ) than seeds of wild-type plants .
	manualset3
131555	5	406588	5	NULL	NULL	0	NULL	salicylic acid-deficient plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Salicylic acid deficiency also improved seed composition in terms of antioxidant vitamin concentrations , seeds of salicylic acid-deficient plants showing higher levels of alpha - and gamma-tocopherol ( vitamin E ) and beta-carotene ( pro-vitamin A ) than seeds of wild-type plants .
	manualset3
131556	6	406588	5	NULL	NULL	0	NULL	higher levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Salicylic acid deficiency also improved seed composition in terms of antioxidant vitamin concentrations , seeds of salicylic acid-deficient plants showing higher levels of alpha - and gamma-tocopherol ( vitamin E ) and beta-carotene ( pro-vitamin A ) than seeds of wild-type plants .
	manualset3
131557	7	406588	5	NULL	NULL	NULL	NULL	alpha - and gamma-tocopherol ( vitamin E )	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Salicylic acid deficiency also improved seed composition in terms of antioxidant vitamin concentrations , seeds of salicylic acid-deficient plants showing higher levels of alpha - and gamma-tocopherol ( vitamin E ) and beta-carotene ( pro-vitamin A ) than seeds of wild-type plants .
	manualset3
131558	8	406588	5	NULL	NULL	0	NULL	 beta-carotene ( pro-vitamin A ) 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Salicylic acid deficiency also improved seed composition in terms of antioxidant vitamin concentrations , seeds of salicylic acid-deficient plants showing higher levels of alpha - and gamma-tocopherol ( vitamin E ) and beta-carotene ( pro-vitamin A ) than seeds of wild-type plants .
	manualset3
131559	9	406588	5	NULL	NULL	0	NULL	seeds 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Salicylic acid deficiency also improved seed composition in terms of antioxidant vitamin concentrations , seeds of salicylic acid-deficient plants showing higher levels of alpha - and gamma-tocopherol ( vitamin E ) and beta-carotene ( pro-vitamin A ) than seeds of wild-type plants .
	manualset3
131560	10	406588	5	NULL	NULL	0	NULL	wild-type plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Salicylic acid deficiency also improved seed composition in terms of antioxidant vitamin concentrations , seeds of salicylic acid-deficient plants showing higher levels of alpha - and gamma-tocopherol ( vitamin E ) and beta-carotene ( pro-vitamin A ) than seeds of wild-type plants .
	manualset3
131561	1	406589	5	NULL	NULL	0	NULL	Salmonella Paratyphi C	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Salmonella Paratyphi C could be differentiated from Salmonella Choleraesuis through the use of primers designed from the viaB gene .
	manualset3
131562	2	406589	5	NULL	NULL	0	NULL	Salmonella Choleraesuis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Salmonella Paratyphi C could be differentiated from Salmonella Choleraesuis through the use of primers designed from the viaB gene .
	manualset3
131563	3	406589	5	NULL	NULL	0	NULL	primers 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Salmonella Paratyphi C could be differentiated from Salmonella Choleraesuis through the use of primers designed from the viaB gene .
	manualset3
131564	4	406589	5	NULL	NULL	0	NULL	viaB gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Salmonella Paratyphi C could be differentiated from Salmonella Choleraesuis through the use of primers designed from the viaB gene .
	manualset3
131565	1	406590	5	NULL	NULL	0	NULL	Salmonella enterica	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Salmonella enterica are Gram-negative enteric pathogens that cause typhoid fever and gastroenteritis in humans .
	manualset3
131566	2	406590	5	NULL	NULL	0	NULL	Gram-negative enteric pathogens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Salmonella enterica are Gram-negative enteric pathogens that cause typhoid fever and gastroenteritis in humans .
	manualset3
131567	3	406590	5	NULL	NULL	0	NULL	typhoid fever	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Salmonella enterica are Gram-negative enteric pathogens that cause typhoid fever and gastroenteritis in humans .
	manualset3
131568	4	406590	5	NULL	NULL	0	NULL	gastroenteritis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Salmonella enterica are Gram-negative enteric pathogens that cause typhoid fever and gastroenteritis in humans .
	manualset3
131569	5	406590	5	NULL	NULL	0	NULL	humans 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Salmonella enterica are Gram-negative enteric pathogens that cause typhoid fever and gastroenteritis in humans .
	manualset3
131570	1	406591	5	NULL	NULL	NULL	NULL	Salmonella enterica serovar London infections	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Salmonella enterica serovar London infections associated with consumption of infant formula .
	manualset3
131571	2	406591	5	NULL	NULL	0	NULL	consumption 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Salmonella enterica serovar London infections associated with consumption of infant formula .
	manualset3
131572	3	406591	5	NULL	NULL	0	NULL	infant formula	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Salmonella enterica serovar London infections associated with consumption of infant formula .
	manualset3
131573	1	406592	5	NULL	NULL	0	NULL	Case 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( Case of hemangio-endothelioma of the breast ) .
	manualset3
131574	2	406592	5	NULL	NULL	0	NULL	hemangio-endothelioma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Case of hemangio-endothelioma of the breast ) .
	manualset3
131575	3	406592	5	NULL	NULL	0	NULL	breast 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Case of hemangio-endothelioma of the breast ) .
	manualset3
131576	1	406593	5	NULL	NULL	0	NULL	desiccant 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A new desiccant consisting of magnesium perchlorate , expanded perlite and metal chelate was prepared .
	manualset3
131577	2	406593	5	NULL	NULL	0	NULL	magnesium perchlorate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A new desiccant consisting of magnesium perchlorate , expanded perlite and metal chelate was prepared .
	manualset3
131578	3	406593	5	NULL	NULL	0	NULL	perlite 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A new desiccant consisting of magnesium perchlorate , expanded perlite and metal chelate was prepared .
	manualset3
131579	4	406593	5	NULL	NULL	0	NULL	metal chelate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A new desiccant consisting of magnesium perchlorate , expanded perlite and metal chelate was prepared .
	manualset3
131580	1	406594	5	NULL	NULL	0	NULL	Salmonella infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Salmonella infection of ovarian dermoid cyst .
	manualset3
131581	2	406594	5	NULL	NULL	0	NULL	ovarian dermoid cyst	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Salmonella infection of ovarian dermoid cyst .
	manualset3
131582	1	406595	5	NULL	NULL	NULL	NULL	Salmonella osteomyelitis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Salmonella osteomyelitis of the tibia treated by a muscle pedicle and delayed bone grafting : a case report .
	manualset3
131583	2	406595	5	NULL	NULL	0	NULL	tibia 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Salmonella osteomyelitis of the tibia treated by a muscle pedicle and delayed bone grafting : a case report .
	manualset3
131584	3	406595	5	NULL	NULL	0	NULL	muscle pedicle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Salmonella osteomyelitis of the tibia treated by a muscle pedicle and delayed bone grafting : a case report .
	manualset3
131585	4	406595	5	NULL	NULL	0	NULL	delayed bone grafting	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Salmonella osteomyelitis of the tibia treated by a muscle pedicle and delayed bone grafting : a case report .
	manualset3
131586	5	406595	5	NULL	NULL	0	NULL	case report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Salmonella osteomyelitis of the tibia treated by a muscle pedicle and delayed bone grafting : a case report .
	manualset3
131587	1	406596	5	NULL	NULL	0	NULL	Salt 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Salt and the development of essential hypertension .
	manualset3
131588	2	406596	5	NULL	NULL	0	NULL	development 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Salt and the development of essential hypertension .
	manualset3
131589	3	406596	5	NULL	NULL	0	NULL	essential hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Salt and the development of essential hypertension .
	manualset3
131590	1	406597	5	NULL	NULL	0	NULL	Salt tolerance 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Salt tolerance of wheat according to soil and drainage water salinity .
	manualset3
131591	2	406597	5	NULL	NULL	0	NULL	wheat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Salt tolerance of wheat according to soil and drainage water salinity .
	manualset3
131592	3	406597	5	NULL	NULL	0	NULL	soil 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Salt tolerance of wheat according to soil and drainage water salinity .
	manualset3
131593	4	406597	5	NULL	NULL	0	NULL	drainage water salinity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Salt tolerance of wheat according to soil and drainage water salinity .
	manualset3
131594	1	406598	5	NULL	NULL	0	NULL	Salvage rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Salvage rates from thrombotic events were unaffected despite rigid flap monitoring protocols .
	manualset3
131595	2	406598	5	NULL	NULL	0	NULL	thrombotic events	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Salvage rates from thrombotic events were unaffected despite rigid flap monitoring protocols .
	manualset3
131596	3	406598	5	NULL	NULL	0	NULL	flap monitoring protocols	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Salvage rates from thrombotic events were unaffected despite rigid flap monitoring protocols .
	manualset3
131597	1	406599	5	NULL	NULL	0	NULL	Sambucus nigra agglutinin ( SNA )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sambucus nigra agglutinin ( SNA ) , which recognizes terminal sialic acids , strongly stained the glandular mucous cells of normal subjects , but not those of patients with chronic sinusitis .
	manualset3
131598	2	406599	5	NULL	NULL	0	NULL	terminal sialic acids	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Sambucus nigra agglutinin ( SNA ) , which recognizes terminal sialic acids , strongly stained the glandular mucous cells of normal subjects , but not those of patients with chronic sinusitis .
	manualset3
131599	3	406599	5	NULL	NULL	0	NULL	glandular mucous cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Sambucus nigra agglutinin ( SNA ) , which recognizes terminal sialic acids , strongly stained the glandular mucous cells of normal subjects , but not those of patients with chronic sinusitis .
	manualset3
131600	4	406599	5	NULL	NULL	0	NULL	normal subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sambucus nigra agglutinin ( SNA ) , which recognizes terminal sialic acids , strongly stained the glandular mucous cells of normal subjects , but not those of patients with chronic sinusitis .
	manualset3
131601	5	406599	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sambucus nigra agglutinin ( SNA ) , which recognizes terminal sialic acids , strongly stained the glandular mucous cells of normal subjects , but not those of patients with chronic sinusitis .
	manualset3
131602	6	406599	5	NULL	NULL	0	NULL	chronic sinusitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Sambucus nigra agglutinin ( SNA ) , which recognizes terminal sialic acids , strongly stained the glandular mucous cells of normal subjects , but not those of patients with chronic sinusitis .
	manualset3
131603	1	406600	5	NULL	NULL	0	NULL	women 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Same women also applied a vehicle control cream to the periorbital skin around the other eye .
	manualset3
131604	2	406600	5	NULL	NULL	0	NULL	vehicle control cream	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Same women also applied a vehicle control cream to the periorbital skin around the other eye .
	manualset3
131605	3	406600	5	NULL	NULL	0	NULL	periorbital skin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Same women also applied a vehicle control cream to the periorbital skin around the other eye .
	manualset3
131606	4	406600	5	NULL	NULL	0	NULL	eye 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Same women also applied a vehicle control cream to the periorbital skin around the other eye .
	manualset3
131607	1	406601	5	NULL	NULL	0	NULL	Sample preparation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sample preparation was investigated using two different stationary phases ( 100 microns polydimethylsiloxane and 85 microns polyacrylate ) , coating a fused silica fiber .
	manualset3
131608	2	406601	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sample preparation was investigated using two different stationary phases ( 100 microns polydimethylsiloxane and 85 microns polyacrylate ) , coating a fused silica fiber .
	manualset3
131609	3	406601	5	NULL	NULL	0	NULL	stationary phases 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sample preparation was investigated using two different stationary phases ( 100 microns polydimethylsiloxane and 85 microns polyacrylate ) , coating a fused silica fiber .
	manualset3
131610	4	406601	5	NULL	NULL	0	NULL	100 microns polydimethylsiloxane	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Sample preparation was investigated using two different stationary phases ( 100 microns polydimethylsiloxane and 85 microns polyacrylate ) , coating a fused silica fiber .
	manualset3
131611	5	406601	5	NULL	NULL	0	NULL	85 microns polyacrylate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Sample preparation was investigated using two different stationary phases ( 100 microns polydimethylsiloxane and 85 microns polyacrylate ) , coating a fused silica fiber .
	manualset3
131612	6	406601	5	NULL	NULL	0	NULL	fused silica fiber	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sample preparation was investigated using two different stationary phases ( 100 microns polydimethylsiloxane and 85 microns polyacrylate ) , coating a fused silica fiber .
	manualset3
131613	1	406602	5	NULL	NULL	0	NULL	Samples 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples from metastatic sites engrafted at higher frequency than those from primary tumors , and stable engraftment of primary tumors in mice correlated with decreased patient survival .
	manualset3
131614	2	406602	5	NULL	NULL	0	NULL	metastatic sites	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples from metastatic sites engrafted at higher frequency than those from primary tumors , and stable engraftment of primary tumors in mice correlated with decreased patient survival .
	manualset3
131615	3	406602	5	NULL	NULL	0	NULL	higher frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples from metastatic sites engrafted at higher frequency than those from primary tumors , and stable engraftment of primary tumors in mice correlated with decreased patient survival .
	manualset3
131616	4	406602	5	NULL	NULL	0	NULL	primary tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples from metastatic sites engrafted at higher frequency than those from primary tumors , and stable engraftment of primary tumors in mice correlated with decreased patient survival .
	manualset3
131617	5	406602	5	NULL	NULL	0	NULL	stable engraftment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples from metastatic sites engrafted at higher frequency than those from primary tumors , and stable engraftment of primary tumors in mice correlated with decreased patient survival .
	manualset3
131618	6	406602	5	NULL	NULL	0	NULL	primary tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples from metastatic sites engrafted at higher frequency than those from primary tumors , and stable engraftment of primary tumors in mice correlated with decreased patient survival .
	manualset3
131619	7	406602	5	NULL	NULL	0	NULL	mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples from metastatic sites engrafted at higher frequency than those from primary tumors , and stable engraftment of primary tumors in mice correlated with decreased patient survival .
	manualset3
131620	8	406602	5	NULL	NULL	0	NULL	patient survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples from metastatic sites engrafted at higher frequency than those from primary tumors , and stable engraftment of primary tumors in mice correlated with decreased patient survival .
	manualset3
131621	1	406603	5	NULL	NULL	0	NULL	Samples 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples of 44 food plants from Bwindi-Impenetrable National Park ( BINP ) and Mgahinga Gorilla National Park ( MGNP ) were tested .
	manualset3
131622	2	406603	5	NULL	NULL	0	NULL	44 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples of 44 food plants from Bwindi-Impenetrable National Park ( BINP ) and Mgahinga Gorilla National Park ( MGNP ) were tested .
	manualset3
131623	3	406603	5	NULL	NULL	0	NULL	food plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples of 44 food plants from Bwindi-Impenetrable National Park ( BINP ) and Mgahinga Gorilla National Park ( MGNP ) were tested .
	manualset3
131624	4	406603	5	NULL	NULL	0	NULL	Bwindi-Impenetrable National Park ( BINP )	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples of 44 food plants from Bwindi-Impenetrable National Park ( BINP ) and Mgahinga Gorilla National Park ( MGNP ) were tested .
	manualset3
131625	5	406603	5	NULL	NULL	0	NULL	Mgahinga Gorilla National Park ( MGNP ) 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples of 44 food plants from Bwindi-Impenetrable National Park ( BINP ) and Mgahinga Gorilla National Park ( MGNP ) were tested .
	manualset3
131626	1	406604	5	NULL	NULL	0	NULL	Samples 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples of air and soil were collected to study the levels of PAHs in the air and soil of the Agra region .
	manualset3
131627	2	406604	5	NULL	NULL	0	NULL	air 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples of air and soil were collected to study the levels of PAHs in the air and soil of the Agra region .
	manualset3
131628	3	406604	5	NULL	NULL	0	NULL	soil 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples of air and soil were collected to study the levels of PAHs in the air and soil of the Agra region .
	manualset3
131629	4	406604	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples of air and soil were collected to study the levels of PAHs in the air and soil of the Agra region .
	manualset3
131630	5	406604	5	NULL	NULL	0	NULL	levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples of air and soil were collected to study the levels of PAHs in the air and soil of the Agra region .
	manualset3
131631	6	406604	5	NULL	NULL	0	NULL	PAHs 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples of air and soil were collected to study the levels of PAHs in the air and soil of the Agra region .
	manualset3
131632	7	406604	5	NULL	NULL	0	NULL	air 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples of air and soil were collected to study the levels of PAHs in the air and soil of the Agra region .
	manualset3
131633	8	406604	5	NULL	NULL	0	NULL	soil 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples of air and soil were collected to study the levels of PAHs in the air and soil of the Agra region .
	manualset3
131634	9	406604	5	NULL	NULL	0	NULL	Agra region	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples of air and soil were collected to study the levels of PAHs in the air and soil of the Agra region .
	manualset3
131635	1	406605	5	NULL	NULL	NULL	NULL	Samples 	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Samples of the secondary uranium minerals collected in the abandoned uranium mine at Pecs ( Hungary ) were investigated by two micro-techniques : scanning electron microscopy ( SEM/EDX ) and micro-Raman spectroscopy ( MRS ) .
	manualset3
131636	2	406605	5	NULL	NULL	0	NULL	secondary uranium minerals 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples of the secondary uranium minerals collected in the abandoned uranium mine at Pecs ( Hungary ) were investigated by two micro-techniques : scanning electron microscopy ( SEM/EDX ) and micro-Raman spectroscopy ( MRS ) .
	manualset3
131637	3	406605	5	NULL	NULL	NULL	NULL	uranium mine	GeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Samples of the secondary uranium minerals collected in the abandoned uranium mine at Pecs ( Hungary ) were investigated by two micro-techniques : scanning electron microscopy ( SEM/EDX ) and micro-Raman spectroscopy ( MRS ) .
	manualset3
131638	4	406605	5	NULL	NULL	0	NULL	Pecs ( Hungary )	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples of the secondary uranium minerals collected in the abandoned uranium mine at Pecs ( Hungary ) were investigated by two micro-techniques : scanning electron microscopy ( SEM/EDX ) and micro-Raman spectroscopy ( MRS ) .
	manualset3
131639	5	406605	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples of the secondary uranium minerals collected in the abandoned uranium mine at Pecs ( Hungary ) were investigated by two micro-techniques : scanning electron microscopy ( SEM/EDX ) and micro-Raman spectroscopy ( MRS ) .
	manualset3
131640	6	406605	5	NULL	NULL	0	NULL	micro-techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples of the secondary uranium minerals collected in the abandoned uranium mine at Pecs ( Hungary ) were investigated by two micro-techniques : scanning electron microscopy ( SEM/EDX ) and micro-Raman spectroscopy ( MRS ) .
	manualset3
131641	7	406605	5	NULL	NULL	0	NULL	scanning electron microscopy ( SEM/EDX )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples of the secondary uranium minerals collected in the abandoned uranium mine at Pecs ( Hungary ) were investigated by two micro-techniques : scanning electron microscopy ( SEM/EDX ) and micro-Raman spectroscopy ( MRS ) .
	manualset3
131642	8	406605	5	NULL	NULL	0	NULL	micro-Raman spectroscopy ( MRS ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples of the secondary uranium minerals collected in the abandoned uranium mine at Pecs ( Hungary ) were investigated by two micro-techniques : scanning electron microscopy ( SEM/EDX ) and micro-Raman spectroscopy ( MRS ) .
	manualset3
131643	1	406606	5	NULL	NULL	0	NULL	Samples 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples were collected from the incubation tubes at various times , extracted with a solid-phase extraction system , and assayed for cocaethylene and 2H5-cocaethylene by GC/MS .
	manualset3
131644	2	406606	5	NULL	NULL	0	NULL	incubation tubes 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples were collected from the incubation tubes at various times , extracted with a solid-phase extraction system , and assayed for cocaethylene and 2H5-cocaethylene by GC/MS .
	manualset3
131645	3	406606	5	NULL	NULL	0	NULL	times 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples were collected from the incubation tubes at various times , extracted with a solid-phase extraction system , and assayed for cocaethylene and 2H5-cocaethylene by GC/MS .
	manualset3
131646	4	406606	5	NULL	NULL	NULL	NULL	solid-phase extraction system 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Samples were collected from the incubation tubes at various times , extracted with a solid-phase extraction system , and assayed for cocaethylene and 2H5-cocaethylene by GC/MS .
	manualset3
131647	5	406606	5	NULL	NULL	0	NULL	cocaethylene 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples were collected from the incubation tubes at various times , extracted with a solid-phase extraction system , and assayed for cocaethylene and 2H5-cocaethylene by GC/MS .
	manualset3
131648	6	406606	5	NULL	NULL	0	NULL	2H5-cocaethylene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples were collected from the incubation tubes at various times , extracted with a solid-phase extraction system , and assayed for cocaethylene and 2H5-cocaethylene by GC/MS .
	manualset3
131649	7	406606	5	NULL	NULL	0	NULL	GC/MS	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples were collected from the incubation tubes at various times , extracted with a solid-phase extraction system , and assayed for cocaethylene and 2H5-cocaethylene by GC/MS .
	manualset3
131650	1	406607	5	NULL	NULL	0	NULL	Samples 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples were screened for the presence of AAV and adenovirus sequences by PCR using degenerate primers .
	manualset3
131651	2	406607	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples were screened for the presence of AAV and adenovirus sequences by PCR using degenerate primers .
	manualset3
131652	3	406607	5	NULL	NULL	NULL	NULL	AAV sequence	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Samples were screened for the presence of AAV and adenovirus sequences by PCR using degenerate primers .
	manualset3
131653	4	406607	5	NULL	NULL	0	NULL	adenovirus sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples were screened for the presence of AAV and adenovirus sequences by PCR using degenerate primers .
	manualset3
131654	5	406607	5	NULL	NULL	0	NULL	adenovirus sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples were screened for the presence of AAV and adenovirus sequences by PCR using degenerate primers .
	manualset3
131655	6	406607	5	NULL	NULL	0	NULL	PCR 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples were screened for the presence of AAV and adenovirus sequences by PCR using degenerate primers .
	manualset3
131656	7	406607	5	NULL	NULL	0	NULL	degenerate primers	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples were screened for the presence of AAV and adenovirus sequences by PCR using degenerate primers .
	manualset3
131657	1	406608	5	NULL	NULL	0	NULL	1 year	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Sampling was conducted for 1 year in a marsh near Buenos Aires from axils of Scirpus giganteus , a larval habitat of the poorly known sabethine mosquito , Isostomyia paranensis .
	manualset3
131658	2	406608	5	NULL	NULL	0	NULL	marsh 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Sampling was conducted for 1 year in a marsh near Buenos Aires from axils of Scirpus giganteus , a larval habitat of the poorly known sabethine mosquito , Isostomyia paranensis .
	manualset3
131659	3	406608	5	NULL	NULL	0	NULL	Buenos Aires	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Sampling was conducted for 1 year in a marsh near Buenos Aires from axils of Scirpus giganteus , a larval habitat of the poorly known sabethine mosquito , Isostomyia paranensis .
	manualset3
131660	4	406608	5	NULL	NULL	0	NULL	axils 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Sampling was conducted for 1 year in a marsh near Buenos Aires from axils of Scirpus giganteus , a larval habitat of the poorly known sabethine mosquito , Isostomyia paranensis .
	manualset3
131661	5	406608	5	NULL	NULL	0	NULL	Scirpus giganteus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sampling was conducted for 1 year in a marsh near Buenos Aires from axils of Scirpus giganteus , a larval habitat of the poorly known sabethine mosquito , Isostomyia paranensis .
	manualset3
131662	6	406608	5	NULL	NULL	0	NULL	larval habitat	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Sampling was conducted for 1 year in a marsh near Buenos Aires from axils of Scirpus giganteus , a larval habitat of the poorly known sabethine mosquito , Isostomyia paranensis .
	manualset3
131663	7	406608	5	NULL	NULL	0	NULL	sabethine mosquito	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sampling was conducted for 1 year in a marsh near Buenos Aires from axils of Scirpus giganteus , a larval habitat of the poorly known sabethine mosquito , Isostomyia paranensis .
	manualset3
131664	8	406608	5	NULL	NULL	0	NULL	Isostomyia paranensis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sampling was conducted for 1 year in a marsh near Buenos Aires from axils of Scirpus giganteus , a larval habitat of the poorly known sabethine mosquito , Isostomyia paranensis .
	manualset3
134861	9	406608	5	NULL	NULL	0	NULL	Sampling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sampling was conducted for 1 year in a marsh near Buenos Aires from axils of Scirpus giganteus , a larval habitat of the poorly known sabethine mosquito , Isostomyia paranensis .
	manualset3
131665	1	406609	5	NULL	NULL	0	NULL	six 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sampling was performed from six locations during biogas production .
	manualset3
131666	2	406609	5	NULL	NULL	0	NULL	locations 	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Sampling was performed from six locations during biogas production .
	manualset3
131667	3	406609	5	NULL	NULL	0	NULL	biogas production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sampling was performed from six locations during biogas production .
	manualset3
131668	1	406610	5	NULL	NULL	0	NULL	esterase variant	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A new esterase variant has been isolated by electrophoresis of homogenized testis , heart , and lung tissues .
	manualset3
131669	2	406610	5	NULL	NULL	0	NULL	electrophoresis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new esterase variant has been isolated by electrophoresis of homogenized testis , heart , and lung tissues .
	manualset3
131670	3	406610	5	NULL	NULL	0	NULL	homogenized testis tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	A new esterase variant has been isolated by electrophoresis of homogenized testis , heart , and lung tissues .
	manualset3
131671	4	406610	5	NULL	NULL	0	NULL	homogenized heart tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	A new esterase variant has been isolated by electrophoresis of homogenized testis , heart , and lung tissues .
	manualset3
131672	5	406610	5	NULL	NULL	0	NULL	homogenized lung tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	A new esterase variant has been isolated by electrophoresis of homogenized testis , heart , and lung tissues .
	manualset3
131673	1	406611	5	NULL	NULL	0	NULL	Sap C	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sap C is responsible for the membrane binding of glucosylceramidase , while Sap A stimulation is possibly related to its effect on the conformation of the enzyme .
	manualset3
131674	2	406611	5	NULL	NULL	0	NULL	membrane binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sap C is responsible for the membrane binding of glucosylceramidase , while Sap A stimulation is possibly related to its effect on the conformation of the enzyme .
	manualset3
131675	3	406611	5	NULL	NULL	0	NULL	glucosylceramidase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sap C is responsible for the membrane binding of glucosylceramidase , while Sap A stimulation is possibly related to its effect on the conformation of the enzyme .
	manualset3
131676	4	406611	5	NULL	NULL	0	NULL	Sap A stimulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sap C is responsible for the membrane binding of glucosylceramidase , while Sap A stimulation is possibly related to its effect on the conformation of the enzyme .
	manualset3
131677	5	406611	5	NULL	NULL	0	NULL	conformation 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sap C is responsible for the membrane binding of glucosylceramidase , while Sap A stimulation is possibly related to its effect on the conformation of the enzyme .
	manualset3
131678	6	406611	5	NULL	NULL	0	NULL	enzyme 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sap C is responsible for the membrane binding of glucosylceramidase , while Sap A stimulation is possibly related to its effect on the conformation of the enzyme .
	manualset3
131679	1	406612	5	NULL	NULL	0	NULL	Sap proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sap proteins fulfill a number of specialized functions during the infective process , which include the simple role of digesting molecules for nutrient acquisition , digesting or distorting host cell membranes to facilitate adhesion and tissue invasion , and digesting cells and molecules of the host immune system to avoid or resist antimicrobial attack by the host .
	manualset3
131680	2	406612	5	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sap proteins fulfill a number of specialized functions during the infective process , which include the simple role of digesting molecules for nutrient acquisition , digesting or distorting host cell membranes to facilitate adhesion and tissue invasion , and digesting cells and molecules of the host immune system to avoid or resist antimicrobial attack by the host .
	manualset3
131681	3	406612	5	NULL	NULL	0	NULL	specialized functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sap proteins fulfill a number of specialized functions during the infective process , which include the simple role of digesting molecules for nutrient acquisition , digesting or distorting host cell membranes to facilitate adhesion and tissue invasion , and digesting cells and molecules of the host immune system to avoid or resist antimicrobial attack by the host .
	manualset3
131682	4	406612	5	NULL	NULL	0	NULL	infective process 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sap proteins fulfill a number of specialized functions during the infective process , which include the simple role of digesting molecules for nutrient acquisition , digesting or distorting host cell membranes to facilitate adhesion and tissue invasion , and digesting cells and molecules of the host immune system to avoid or resist antimicrobial attack by the host .
	manualset3
131683	5	406612	5	NULL	NULL	0	NULL	simple role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sap proteins fulfill a number of specialized functions during the infective process , which include the simple role of digesting molecules for nutrient acquisition , digesting or distorting host cell membranes to facilitate adhesion and tissue invasion , and digesting cells and molecules of the host immune system to avoid or resist antimicrobial attack by the host .
	manualset3
131684	6	406612	5	NULL	NULL	0	NULL	molecules 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Sap proteins fulfill a number of specialized functions during the infective process , which include the simple role of digesting molecules for nutrient acquisition , digesting or distorting host cell membranes to facilitate adhesion and tissue invasion , and digesting cells and molecules of the host immune system to avoid or resist antimicrobial attack by the host .
	manualset3
131685	7	406612	5	NULL	NULL	0	NULL	nutrient acquisition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sap proteins fulfill a number of specialized functions during the infective process , which include the simple role of digesting molecules for nutrient acquisition , digesting or distorting host cell membranes to facilitate adhesion and tissue invasion , and digesting cells and molecules of the host immune system to avoid or resist antimicrobial attack by the host .
	manualset3
131686	8	406612	5	NULL	NULL	0	NULL	host cell membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Sap proteins fulfill a number of specialized functions during the infective process , which include the simple role of digesting molecules for nutrient acquisition , digesting or distorting host cell membranes to facilitate adhesion and tissue invasion , and digesting cells and molecules of the host immune system to avoid or resist antimicrobial attack by the host .
	manualset3
131687	9	406612	5	NULL	NULL	0	NULL	adhesion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sap proteins fulfill a number of specialized functions during the infective process , which include the simple role of digesting molecules for nutrient acquisition , digesting or distorting host cell membranes to facilitate adhesion and tissue invasion , and digesting cells and molecules of the host immune system to avoid or resist antimicrobial attack by the host .
	manualset3
131688	10	406612	5	NULL	NULL	0	NULL	tissue invasion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sap proteins fulfill a number of specialized functions during the infective process , which include the simple role of digesting molecules for nutrient acquisition , digesting or distorting host cell membranes to facilitate adhesion and tissue invasion , and digesting cells and molecules of the host immune system to avoid or resist antimicrobial attack by the host .
	manualset3
131689	11	406612	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Sap proteins fulfill a number of specialized functions during the infective process , which include the simple role of digesting molecules for nutrient acquisition , digesting or distorting host cell membranes to facilitate adhesion and tissue invasion , and digesting cells and molecules of the host immune system to avoid or resist antimicrobial attack by the host .
	manualset3
131690	12	406612	5	NULL	NULL	0	NULL	molecules 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Sap proteins fulfill a number of specialized functions during the infective process , which include the simple role of digesting molecules for nutrient acquisition , digesting or distorting host cell membranes to facilitate adhesion and tissue invasion , and digesting cells and molecules of the host immune system to avoid or resist antimicrobial attack by the host .
	manualset3
131691	13	406612	5	NULL	NULL	NULL	NULL	host immune system	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Sap proteins fulfill a number of specialized functions during the infective process , which include the simple role of digesting molecules for nutrient acquisition , digesting or distorting host cell membranes to facilitate adhesion and tissue invasion , and digesting cells and molecules of the host immune system to avoid or resist antimicrobial attack by the host .
	manualset3
131692	14	406612	5	NULL	NULL	0	NULL	antimicrobial attack	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sap proteins fulfill a number of specialized functions during the infective process , which include the simple role of digesting molecules for nutrient acquisition , digesting or distorting host cell membranes to facilitate adhesion and tissue invasion , and digesting cells and molecules of the host immune system to avoid or resist antimicrobial attack by the host .
	manualset3
131693	15	406612	5	NULL	NULL	0	NULL	host 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sap proteins fulfill a number of specialized functions during the infective process , which include the simple role of digesting molecules for nutrient acquisition , digesting or distorting host cell membranes to facilitate adhesion and tissue invasion , and digesting cells and molecules of the host immune system to avoid or resist antimicrobial attack by the host .
	manualset3
131694	1	406613	5	NULL	NULL	0	NULL	Sarcocysts	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Sarcocysts of S. inghami are also described .
	manualset3
131695	2	406613	5	NULL	NULL	0	NULL	 S. inghami	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sarcocysts of S. inghami are also described .
	manualset3
131696	1	406614	5	NULL	NULL	0	NULL	Sarcoidosis ( SAR )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Sarcoidosis ( SAR ) is a systemic granulomatous inflammatory disease characterized by recruitment and activation of peripheral blood mononuclear cells to the sites of disease .
	manualset3
131697	2	406614	5	NULL	NULL	0	NULL	systemic granulomatous inflammatory disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Sarcoidosis ( SAR ) is a systemic granulomatous inflammatory disease characterized by recruitment and activation of peripheral blood mononuclear cells to the sites of disease .
	manualset3
131698	3	406614	5	NULL	NULL	0	NULL	recruitment 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sarcoidosis ( SAR ) is a systemic granulomatous inflammatory disease characterized by recruitment and activation of peripheral blood mononuclear cells to the sites of disease .
	manualset3
131699	4	406614	5	NULL	NULL	0	NULL	activation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sarcoidosis ( SAR ) is a systemic granulomatous inflammatory disease characterized by recruitment and activation of peripheral blood mononuclear cells to the sites of disease .
	manualset3
131700	5	406614	5	NULL	NULL	0	NULL	peripheral blood mononuclear cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Sarcoidosis ( SAR ) is a systemic granulomatous inflammatory disease characterized by recruitment and activation of peripheral blood mononuclear cells to the sites of disease .
	manualset3
131701	6	406614	5	NULL	NULL	NULL	NULL	sites of disease	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Sarcoidosis ( SAR ) is a systemic granulomatous inflammatory disease characterized by recruitment and activation of peripheral blood mononuclear cells to the sites of disease .
	manualset3
131702	1	406615	5	NULL	NULL	0	NULL	Satellite clinics	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Satellite clinics enhance reach and reputation : it 's all about customer service in West Bend , Wisconsin .
	manualset3
131703	2	406615	5	NULL	NULL	0	NULL	reputation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Satellite clinics enhance reach and reputation : it 's all about customer service in West Bend , Wisconsin .
	manualset3
131704	3	406615	5	NULL	NULL	0	NULL	customer service	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Satellite clinics enhance reach and reputation : it 's all about customer service in West Bend , Wisconsin .
	manualset3
131705	4	406615	5	NULL	NULL	0	NULL	West Bend , Wisconsin	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Satellite clinics enhance reach and reputation : it 's all about customer service in West Bend , Wisconsin .
	manualset3
131706	1	406616	5	NULL	NULL	0	NULL	ethic 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new ethic for medicine and society .
	manualset3
131707	2	406616	5	NULL	NULL	0	NULL	medicine 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new ethic for medicine and society .
	manualset3
131708	3	406616	5	NULL	NULL	0	NULL	society 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A new ethic for medicine and society .
	manualset3
131709	1	406617	5	NULL	NULL	0	NULL	Saturation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Saturation of influx and efflux occurs .
	manualset3
131710	2	406617	5	NULL	NULL	0	NULL	influx 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Saturation of influx and efflux occurs .
	manualset3
131711	3	406617	5	NULL	NULL	0	NULL	efflux 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Saturation of influx and efflux occurs .
	manualset3
131712	1	406618	5	NULL	NULL	0	NULL	Scalar coupling constants	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Scalar coupling constants for the sugar protons were determined by quantitative simulations of DQF-COSY cross-peaks and used to determine sugar pucker populations .
	manualset3
131713	2	406618	5	NULL	NULL	0	NULL	sugar protons	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Scalar coupling constants for the sugar protons were determined by quantitative simulations of DQF-COSY cross-peaks and used to determine sugar pucker populations .
	manualset3
131714	3	406618	5	NULL	NULL	0	NULL	quantitative simulations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Scalar coupling constants for the sugar protons were determined by quantitative simulations of DQF-COSY cross-peaks and used to determine sugar pucker populations .
	manualset3
131715	4	406618	5	NULL	NULL	0	NULL	DQF-COSY cross-peaks	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Scalar coupling constants for the sugar protons were determined by quantitative simulations of DQF-COSY cross-peaks and used to determine sugar pucker populations .
	manualset3
131716	5	406618	5	NULL	NULL	0	NULL	sugar pucker populations	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Scalar coupling constants for the sugar protons were determined by quantitative simulations of DQF-COSY cross-peaks and used to determine sugar pucker populations .
	manualset3
131717	1	406619	5	NULL	NULL	0	NULL	Scalar timing	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Scalar timing in temporal generalization in children with short and long stimulus durations .
	manualset3
131718	2	406619	5	NULL	NULL	0	NULL	temporal generalization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Scalar timing in temporal generalization in children with short and long stimulus durations .
	manualset3
131719	3	406619	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Scalar timing in temporal generalization in children with short and long stimulus durations .
	manualset3
131720	4	406619	5	NULL	NULL	0	NULL	short stimulus durations	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Scalar timing in temporal generalization in children with short and long stimulus durations .
	manualset3
131721	5	406619	5	NULL	NULL	0	NULL	long stimulus durations	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Scalar timing in temporal generalization in children with short and long stimulus durations .
	manualset3
131722	1	406620	5	NULL	NULL	0	NULL	Scale-up	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Scale-up for bulk production of vaccine against meningococcal disease .
	manualset3
131723	2	406620	5	NULL	NULL	0	NULL	bulk production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Scale-up for bulk production of vaccine against meningococcal disease .
	manualset3
131724	3	406620	5	NULL	NULL	0	NULL	vaccine 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Scale-up for bulk production of vaccine against meningococcal disease .
	manualset3
131725	4	406620	5	NULL	NULL	0	NULL	meningococcal disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Scale-up for bulk production of vaccine against meningococcal disease .
	manualset3
131726	1	406621	5	NULL	NULL	0	NULL	Scanning electron microscopy ( SEM )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Scanning electron microscopy ( SEM ) has shown one change of particle between 2 microm at 90 microm and apparent porosity , thermal analysis has shown loss of mass and residual decomposition in the TG , DTG and DTA curves .
	manualset3
131727	2	406621	5	NULL	NULL	0	NULL	one 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Scanning electron microscopy ( SEM ) has shown one change of particle between 2 microm at 90 microm and apparent porosity , thermal analysis has shown loss of mass and residual decomposition in the TG , DTG and DTA curves .
	manualset3
131728	3	406621	5	NULL	NULL	0	NULL	particle 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Scanning electron microscopy ( SEM ) has shown one change of particle between 2 microm at 90 microm and apparent porosity , thermal analysis has shown loss of mass and residual decomposition in the TG , DTG and DTA curves .
	manualset3
131729	4	406621	5	NULL	NULL	0	NULL	2 microm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Scanning electron microscopy ( SEM ) has shown one change of particle between 2 microm at 90 microm and apparent porosity , thermal analysis has shown loss of mass and residual decomposition in the TG , DTG and DTA curves .
	manualset3
131730	5	406621	5	NULL	NULL	0	NULL	90 microm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Scanning electron microscopy ( SEM ) has shown one change of particle between 2 microm at 90 microm and apparent porosity , thermal analysis has shown loss of mass and residual decomposition in the TG , DTG and DTA curves .
	manualset3
131731	6	406621	5	NULL	NULL	0	NULL	apparent porosity 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Scanning electron microscopy ( SEM ) has shown one change of particle between 2 microm at 90 microm and apparent porosity , thermal analysis has shown loss of mass and residual decomposition in the TG , DTG and DTA curves .
	manualset3
131733	7	406621	5	NULL	NULL	0	NULL	thermal analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Scanning electron microscopy ( SEM ) has shown one change of particle between 2 microm at 90 microm and apparent porosity , thermal analysis has shown loss of mass and residual decomposition in the TG , DTG and DTA curves .
	manualset3
131734	8	406621	5	NULL	NULL	0	NULL	mass 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Scanning electron microscopy ( SEM ) has shown one change of particle between 2 microm at 90 microm and apparent porosity , thermal analysis has shown loss of mass and residual decomposition in the TG , DTG and DTA curves .
	manualset3
131735	9	406621	5	NULL	NULL	0	NULL	residual decomposition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Scanning electron microscopy ( SEM ) has shown one change of particle between 2 microm at 90 microm and apparent porosity , thermal analysis has shown loss of mass and residual decomposition in the TG , DTG and DTA curves .
	manualset3
131736	10	406621	5	NULL	NULL	0	NULL	TG curve	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Scanning electron microscopy ( SEM ) has shown one change of particle between 2 microm at 90 microm and apparent porosity , thermal analysis has shown loss of mass and residual decomposition in the TG , DTG and DTA curves .
	manualset3
131737	11	406621	5	NULL	NULL	0	NULL	DTG curve	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Scanning electron microscopy ( SEM ) has shown one change of particle between 2 microm at 90 microm and apparent porosity , thermal analysis has shown loss of mass and residual decomposition in the TG , DTG and DTA curves .
	manualset3
131738	12	406621	5	NULL	NULL	0	NULL	DTA curve	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Scanning electron microscopy ( SEM ) has shown one change of particle between 2 microm at 90 microm and apparent porosity , thermal analysis has shown loss of mass and residual decomposition in the TG , DTG and DTA curves .
	manualset3
131739	1	406622	5	NULL	NULL	0	NULL	facile method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A new facile method for spin-labeling of oligonucleotides .
	manualset3
131740	2	406622	5	NULL	NULL	0	NULL	oligonucleotides 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A new facile method for spin-labeling of oligonucleotides .
	manualset3
134862	3	406622	5	NULL	NULL	0	NULL	 spin-labeling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new facile method for spin-labeling of oligonucleotides .
	manualset3
131741	1	406623	5	NULL	NULL	0	NULL	Schiff bases 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Schiff bases as potential fungicides and nitrification inhibitors .
	manualset3
131742	2	406623	5	NULL	NULL	0	NULL	potential fungicides 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Schiff bases as potential fungicides and nitrification inhibitors .
	manualset3
131743	3	406623	5	NULL	NULL	0	NULL	nitrification inhibitors 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Schiff bases as potential fungicides and nitrification inhibitors .
	manualset3
131744	1	406624	5	NULL	NULL	0	NULL	Schistosomal glomerulopathy 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Schistosomal glomerulopathy and changes in the distribution of histological patterns of glomerular diseases in Bahia , Brazil .
	manualset3
131745	2	406624	5	NULL	NULL	0	NULL	distribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Schistosomal glomerulopathy and changes in the distribution of histological patterns of glomerular diseases in Bahia , Brazil .
	manualset3
131746	3	406624	5	NULL	NULL	0	NULL	histological patterns	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Schistosomal glomerulopathy and changes in the distribution of histological patterns of glomerular diseases in Bahia , Brazil .
	manualset3
131747	4	406624	5	NULL	NULL	0	NULL	glomerular diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Schistosomal glomerulopathy and changes in the distribution of histological patterns of glomerular diseases in Bahia , Brazil .
	manualset3
131748	5	406624	5	NULL	NULL	0	NULL	Bahia , Brazil 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Schistosomal glomerulopathy and changes in the distribution of histological patterns of glomerular diseases in Bahia , Brazil .
	manualset3
131749	1	406625	5	NULL	NULL	0	NULL	Schistosomiasis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Schistosomiasis : from drug deployment to drug development .
	manualset3
131750	2	406625	5	NULL	NULL	0	NULL	drug deployment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Schistosomiasis : from drug deployment to drug development .
	manualset3
131751	3	406625	5	NULL	NULL	0	NULL	drug development	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Schistosomiasis : from drug deployment to drug development .
	manualset3
131752	1	406626	5	NULL	NULL	0	NULL	Schizophrenia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Schizophrenia is a severe mental illness characterized by behavioral and cognitive symptoms .
	manualset3
131753	2	406626	5	NULL	NULL	0	NULL	severe mental illness	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Schizophrenia is a severe mental illness characterized by behavioral and cognitive symptoms .
	manualset3
131754	3	406626	5	NULL	NULL	0	NULL	behavioral symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Schizophrenia is a severe mental illness characterized by behavioral and cognitive symptoms .
	manualset3
131755	4	406626	5	NULL	NULL	0	NULL	cognitive symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Schizophrenia is a severe mental illness characterized by behavioral and cognitive symptoms .
	manualset3
131756	1	406627	5	NULL	NULL	0	NULL	Schizophrenics 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Schizophrenics have deficits in neuropsychological performance , some of which are modified by cigarette smoking .
	manualset3
131757	2	406627	5	NULL	NULL	0	NULL	deficits 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Schizophrenics have deficits in neuropsychological performance , some of which are modified by cigarette smoking .
	manualset3
131758	3	406627	5	NULL	NULL	0	NULL	neuropsychological performance	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Schizophrenics have deficits in neuropsychological performance , some of which are modified by cigarette smoking .
	manualset3
131759	4	406627	5	NULL	NULL	0	NULL	cigarette smoking	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Schizophrenics have deficits in neuropsychological performance , some of which are modified by cigarette smoking .
	manualset3
131760	1	406628	5	NULL	NULL	0	NULL	Scientific validation procedures 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Scientific validation procedures should be applied to the classification of depressions , including studies of natural history and course , specific antidepressant drug responses , and the use of laboratory markers such as the dexamethasone suppression test and sleep EEG parameters .
	manualset3
131761	2	406628	5	NULL	NULL	0	NULL	classification 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Scientific validation procedures should be applied to the classification of depressions , including studies of natural history and course , specific antidepressant drug responses , and the use of laboratory markers such as the dexamethasone suppression test and sleep EEG parameters .
	manualset3
131762	3	406628	5	NULL	NULL	0	NULL	depressions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Scientific validation procedures should be applied to the classification of depressions , including studies of natural history and course , specific antidepressant drug responses , and the use of laboratory markers such as the dexamethasone suppression test and sleep EEG parameters .
	manualset3
131763	4	406628	5	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Scientific validation procedures should be applied to the classification of depressions , including studies of natural history and course , specific antidepressant drug responses , and the use of laboratory markers such as the dexamethasone suppression test and sleep EEG parameters .
	manualset3
131764	5	406628	5	NULL	NULL	0	NULL	natural history	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Scientific validation procedures should be applied to the classification of depressions , including studies of natural history and course , specific antidepressant drug responses , and the use of laboratory markers such as the dexamethasone suppression test and sleep EEG parameters .
	manualset3
131765	6	406628	5	NULL	NULL	0	NULL	course 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Scientific validation procedures should be applied to the classification of depressions , including studies of natural history and course , specific antidepressant drug responses , and the use of laboratory markers such as the dexamethasone suppression test and sleep EEG parameters .
	manualset3
131766	7	406628	5	NULL	NULL	0	NULL	specific antidepressant drug responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Scientific validation procedures should be applied to the classification of depressions , including studies of natural history and course , specific antidepressant drug responses , and the use of laboratory markers such as the dexamethasone suppression test and sleep EEG parameters .
	manualset3
131767	8	406628	5	NULL	NULL	NULL	NULL	laboratory markers	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Scientific validation procedures should be applied to the classification of depressions , including studies of natural history and course , specific antidepressant drug responses , and the use of laboratory markers such as the dexamethasone suppression test and sleep EEG parameters .
	manualset3
131768	9	406628	5	NULL	NULL	0	NULL	dexamethasone suppression test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Scientific validation procedures should be applied to the classification of depressions , including studies of natural history and course , specific antidepressant drug responses , and the use of laboratory markers such as the dexamethasone suppression test and sleep EEG parameters .
	manualset3
131769	10	406628	5	NULL	NULL	0	NULL	sleep EEG parameters	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Scientific validation procedures should be applied to the classification of depressions , including studies of natural history and course , specific antidepressant drug responses , and the use of laboratory markers such as the dexamethasone suppression test and sleep EEG parameters .
	manualset3
131770	1	406629	5	NULL	NULL	0	NULL	Scleroedema adultorum	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Scleroedema adultorum associated with sarcoidosis .
	manualset3
131771	2	406629	5	NULL	NULL	0	NULL	sarcoidosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Scleroedema adultorum associated with sarcoidosis .
	manualset3
131772	1	406630	5	NULL	NULL	0	NULL	Scleromyxedema 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Scleromyxedema is an unusual skin disease that is characterized by a proliferation of fibroblasts and an accumulation of mucin .
	manualset3
131773	2	406630	5	NULL	NULL	0	NULL	unusual skin disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Scleromyxedema is an unusual skin disease that is characterized by a proliferation of fibroblasts and an accumulation of mucin .
	manualset3
131774	3	406630	5	NULL	NULL	0	NULL	proliferation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Scleromyxedema is an unusual skin disease that is characterized by a proliferation of fibroblasts and an accumulation of mucin .
	manualset3
131775	4	406630	5	NULL	NULL	0	NULL	fibroblasts 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Scleromyxedema is an unusual skin disease that is characterized by a proliferation of fibroblasts and an accumulation of mucin .
	manualset3
131776	5	406630	5	NULL	NULL	0	NULL	accumulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Scleromyxedema is an unusual skin disease that is characterized by a proliferation of fibroblasts and an accumulation of mucin .
	manualset3
131777	6	406630	5	NULL	NULL	0	NULL	mucin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Scleromyxedema is an unusual skin disease that is characterized by a proliferation of fibroblasts and an accumulation of mucin .
	manualset3
132134	1	406631	5	NULL	NULL	0	NULL	Scopolamine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Scopolamine ( 4-32 micrograms/kg , SC ) selectively decreased the CR % for delayed trials in five out of eight animals , suggesting impairment of short-term memory .
	manualset3
132135	2	406631	5	NULL	NULL	0	NULL	4-32 micrograms/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Scopolamine ( 4-32 micrograms/kg , SC ) selectively decreased the CR % for delayed trials in five out of eight animals , suggesting impairment of short-term memory .
	manualset3
132136	3	406631	5	NULL	NULL	0	NULL	CR %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Scopolamine ( 4-32 micrograms/kg , SC ) selectively decreased the CR % for delayed trials in five out of eight animals , suggesting impairment of short-term memory .
	manualset3
132137	4	406631	5	NULL	NULL	0	NULL	delayed trials	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Scopolamine ( 4-32 micrograms/kg , SC ) selectively decreased the CR % for delayed trials in five out of eight animals , suggesting impairment of short-term memory .
	manualset3
132138	5	406631	5	NULL	NULL	0	NULL	five out of eight	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Scopolamine ( 4-32 micrograms/kg , SC ) selectively decreased the CR % for delayed trials in five out of eight animals , suggesting impairment of short-term memory .
	manualset3
132139	6	406631	5	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Scopolamine ( 4-32 micrograms/kg , SC ) selectively decreased the CR % for delayed trials in five out of eight animals , suggesting impairment of short-term memory .
	manualset3
132140	7	406631	5	NULL	NULL	0	NULL	impairment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Scopolamine ( 4-32 micrograms/kg , SC ) selectively decreased the CR % for delayed trials in five out of eight animals , suggesting impairment of short-term memory .
	manualset3
132141	8	406631	5	NULL	NULL	0	NULL	short-term memory	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Scopolamine ( 4-32 micrograms/kg , SC ) selectively decreased the CR % for delayed trials in five out of eight animals , suggesting impairment of short-term memory .
	manualset3
132142	1	406632	5	NULL	NULL	NULL	NULL	Scott	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Scott and his family denied a history of prodromal symptoms , mental or medical illnesses , including head injury .
	manualset3
132143	2	406632	5	NULL	NULL	0	NULL	family	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Scott and his family denied a history of prodromal symptoms , mental or medical illnesses , including head injury .
	manualset3
132144	3	406632	5	NULL	NULL	0	NULL	history	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Scott and his family denied a history of prodromal symptoms , mental or medical illnesses , including head injury .
	manualset3
132145	4	406632	5	NULL	NULL	0	NULL	prodromal symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Scott and his family denied a history of prodromal symptoms , mental or medical illnesses , including head injury .
	manualset3
132146	5	406632	5	NULL	NULL	0	NULL	mental or medical illnesses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Scott and his family denied a history of prodromal symptoms , mental or medical illnesses , including head injury .
	manualset3
132147	6	406632	5	NULL	NULL	0	NULL	head injury 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Scott and his family denied a history of prodromal symptoms , mental or medical illnesses , including head injury .
	manualset3
132148	1	406633	5	NULL	NULL	0	NULL	new form of vascular congestion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A new form of vascular congestion : Crowded right atrium during new device procedures .
	manualset3
132149	2	406633	5	NULL	NULL	0	NULL	right atrium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A new form of vascular congestion : Crowded right atrium during new device procedures .
	manualset3
132150	3	406633	5	NULL	NULL	0	NULL	new device procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A new form of vascular congestion : Crowded right atrium during new device procedures .
	manualset3
132151	1	406634	5	NULL	NULL	0	NULL	Screening	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Screening for fetal urological abnormalities : how effective ?
	manualset3
132152	2	406634	5	NULL	NULL	0	NULL	fetal urological abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Screening for fetal urological abnormalities : how effective ?
	manualset3
132153	1	406635	5	NULL	NULL	0	NULL	Screening tools	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Screening tools for psychological distress and patient question prompt sheets administered prior to the consultation can also be useful .
	manualset3
132154	2	406635	5	NULL	NULL	0	NULL	psychological distress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Screening tools for psychological distress and patient question prompt sheets administered prior to the consultation can also be useful .
	manualset3
132155	3	406635	5	NULL	NULL	0	NULL	patient question prompt sheets	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Screening tools for psychological distress and patient question prompt sheets administered prior to the consultation can also be useful .
	manualset3
132156	4	406635	5	NULL	NULL	0	NULL	consultation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Screening tools for psychological distress and patient question prompt sheets administered prior to the consultation can also be useful .
	manualset3
132157	1	406636	5	NULL	NULL	0	NULL	Screens	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Screens to update patients in emergency departments about their progress can help to reduce aggression .
	manualset3
132158	2	406636	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Screens to update patients in emergency departments about their progress can help to reduce aggression .
	manualset3
132159	3	406636	5	NULL	NULL	0	NULL	emergency departments	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Screens to update patients in emergency departments about their progress can help to reduce aggression .
	manualset3
132160	4	406636	5	NULL	NULL	0	NULL	aggression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Screens to update patients in emergency departments about their progress can help to reduce aggression .
	manualset3
134863	5	406636	5	NULL	NULL	0	NULL	progress 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Screens to update patients in emergency departments about their progress can help to reduce aggression .
	manualset3
132161	1	406637	5	NULL	NULL	0	NULL	Scutellarein	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Scutellarein and nepetin were found to be inhibitors of xanthine oxidase activity , whereas morelloflavone acted as a scavenger of superoxide generated by hypoxanthine/xanthine oxidase .
	manualset3
132162	2	406637	5	NULL	NULL	0	NULL	nepetin	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Scutellarein and nepetin were found to be inhibitors of xanthine oxidase activity , whereas morelloflavone acted as a scavenger of superoxide generated by hypoxanthine/xanthine oxidase .
	manualset3
132163	3	406637	5	NULL	NULL	0	NULL	inhibitors	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Scutellarein and nepetin were found to be inhibitors of xanthine oxidase activity , whereas morelloflavone acted as a scavenger of superoxide generated by hypoxanthine/xanthine oxidase .
	manualset3
132164	4	406637	5	NULL	NULL	0	NULL	 xanthine oxidase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Scutellarein and nepetin were found to be inhibitors of xanthine oxidase activity , whereas morelloflavone acted as a scavenger of superoxide generated by hypoxanthine/xanthine oxidase .
	manualset3
132165	5	406637	5	NULL	NULL	0	NULL	morelloflavone	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Scutellarein and nepetin were found to be inhibitors of xanthine oxidase activity , whereas morelloflavone acted as a scavenger of superoxide generated by hypoxanthine/xanthine oxidase .
	manualset3
132166	6	406637	5	NULL	NULL	0	NULL	scavenger	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Scutellarein and nepetin were found to be inhibitors of xanthine oxidase activity , whereas morelloflavone acted as a scavenger of superoxide generated by hypoxanthine/xanthine oxidase .
	manualset3
132167	7	406637	5	NULL	NULL	0	NULL	superoxide	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Scutellarein and nepetin were found to be inhibitors of xanthine oxidase activity , whereas morelloflavone acted as a scavenger of superoxide generated by hypoxanthine/xanthine oxidase .
	manualset3
132168	8	406637	5	NULL	NULL	NULL	NULL	hypoxanthine/xanthine oxidase	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Scutellarein and nepetin were found to be inhibitors of xanthine oxidase activity , whereas morelloflavone acted as a scavenger of superoxide generated by hypoxanthine/xanthine oxidase .
	manualset3
132169	1	406638	5	NULL	NULL	0	NULL	Se-deficient Hubbard chicks	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Se-deficient Hubbard chicks , on the other hand , gained faster and more efficiently when fed the Met-Cys-Cys combination than when fed an isosulfurous level of Met alone .
	manualset3
132170	2	406638	5	NULL	NULL	0	NULL	Met-Cys-Cys combination	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Se-deficient Hubbard chicks , on the other hand , gained faster and more efficiently when fed the Met-Cys-Cys combination than when fed an isosulfurous level of Met alone .
	manualset3
132171	3	406638	5	NULL	NULL	0	NULL	isosulfurous level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Se-deficient Hubbard chicks , on the other hand , gained faster and more efficiently when fed the Met-Cys-Cys combination than when fed an isosulfurous level of Met alone .
	manualset3
132172	4	406638	5	NULL	NULL	0	NULL	Met	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Se-deficient Hubbard chicks , on the other hand , gained faster and more efficiently when fed the Met-Cys-Cys combination than when fed an isosulfurous level of Met alone .
	manualset3
132173	1	406639	5	NULL	NULL	0	NULL	Sea urchin embryos	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sea urchin embryos as a model system for studying autophagy induced by cadmium stress .
	manualset3
132174	2	406639	5	NULL	NULL	0	NULL	model system	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Sea urchin embryos as a model system for studying autophagy induced by cadmium stress .
	manualset3
132175	3	406639	5	NULL	NULL	0	NULL	autophagy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sea urchin embryos as a model system for studying autophagy induced by cadmium stress .
	manualset3
132176	4	406639	5	NULL	NULL	0	NULL	cadmium stress	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sea urchin embryos as a model system for studying autophagy induced by cadmium stress .
	manualset3
132177	1	406640	5	NULL	NULL	0	NULL	Search terms	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Search terms were nursing shortage , job satisfaction in nursing , stress in nursing , nursing turnover , nursing image , nursing work environment , physical demands of nursing , and nursing faculty shortage .
	manualset3
132178	2	406640	5	NULL	NULL	0	NULL	nursing shortage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Search terms were nursing shortage , job satisfaction in nursing , stress in nursing , nursing turnover , nursing image , nursing work environment , physical demands of nursing , and nursing faculty shortage .
	manualset3
132179	3	406640	5	NULL	NULL	0	NULL	job satisfaction	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Search terms were nursing shortage , job satisfaction in nursing , stress in nursing , nursing turnover , nursing image , nursing work environment , physical demands of nursing , and nursing faculty shortage .
	manualset3
132180	4	406640	5	NULL	NULL	0	NULL	nursing	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Search terms were nursing shortage , job satisfaction in nursing , stress in nursing , nursing turnover , nursing image , nursing work environment , physical demands of nursing , and nursing faculty shortage .
	manualset3
132181	5	406640	5	NULL	NULL	0	NULL	stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Search terms were nursing shortage , job satisfaction in nursing , stress in nursing , nursing turnover , nursing image , nursing work environment , physical demands of nursing , and nursing faculty shortage .
	manualset3
132182	6	406640	5	NULL	NULL	0	NULL	nursing	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Search terms were nursing shortage , job satisfaction in nursing , stress in nursing , nursing turnover , nursing image , nursing work environment , physical demands of nursing , and nursing faculty shortage .
	manualset3
132183	7	406640	5	NULL	NULL	0	NULL	nursing turnover	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Search terms were nursing shortage , job satisfaction in nursing , stress in nursing , nursing turnover , nursing image , nursing work environment , physical demands of nursing , and nursing faculty shortage .
	manualset3
132184	8	406640	5	NULL	NULL	0	NULL	nursing image	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Search terms were nursing shortage , job satisfaction in nursing , stress in nursing , nursing turnover , nursing image , nursing work environment , physical demands of nursing , and nursing faculty shortage .
	manualset3
132185	9	406640	5	NULL	NULL	0	NULL	nursing work environment	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Search terms were nursing shortage , job satisfaction in nursing , stress in nursing , nursing turnover , nursing image , nursing work environment , physical demands of nursing , and nursing faculty shortage .
	manualset3
132186	10	406640	5	NULL	NULL	0	NULL	physical demands	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Search terms were nursing shortage , job satisfaction in nursing , stress in nursing , nursing turnover , nursing image , nursing work environment , physical demands of nursing , and nursing faculty shortage .
	manualset3
132187	11	406640	5	NULL	NULL	0	NULL	nursing	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Search terms were nursing shortage , job satisfaction in nursing , stress in nursing , nursing turnover , nursing image , nursing work environment , physical demands of nursing , and nursing faculty shortage .
	manualset3
132188	12	406640	5	NULL	NULL	0	NULL	nursing faculty shortage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Search terms were nursing shortage , job satisfaction in nursing , stress in nursing , nursing turnover , nursing image , nursing work environment , physical demands of nursing , and nursing faculty shortage .
	manualset3
132189	1	406641	5	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Searching for genes involved in arteriosclerosis : proteomic analysis of cultured human umbilical vein endothelial cells undergoing replicative senescence .
	manualset3
132190	2	406641	5	NULL	NULL	0	NULL	arteriosclerosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Searching for genes involved in arteriosclerosis : proteomic analysis of cultured human umbilical vein endothelial cells undergoing replicative senescence .
	manualset3
132191	3	406641	5	NULL	NULL	0	NULL	proteomic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Searching for genes involved in arteriosclerosis : proteomic analysis of cultured human umbilical vein endothelial cells undergoing replicative senescence .
	manualset3
132192	4	406641	5	NULL	NULL	0	NULL	cultured human umbilical vein endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Searching for genes involved in arteriosclerosis : proteomic analysis of cultured human umbilical vein endothelial cells undergoing replicative senescence .
	manualset3
132193	5	406641	5	NULL	NULL	0	NULL	replicative senescence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Searching for genes involved in arteriosclerosis : proteomic analysis of cultured human umbilical vein endothelial cells undergoing replicative senescence .
	manualset3
132194	1	406642	5	NULL	NULL	0	NULL	hierarchical key	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new hierarchical key for the identification of triacyl quinic acids is presented , based on previously established rules of fragmentation .
	manualset3
132195	2	406642	5	NULL	NULL	0	NULL	identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A new hierarchical key for the identification of triacyl quinic acids is presented , based on previously established rules of fragmentation .
	manualset3
132196	3	406642	5	NULL	NULL	0	NULL	triacyl quinic acids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A new hierarchical key for the identification of triacyl quinic acids is presented , based on previously established rules of fragmentation .
	manualset3
132197	4	406642	5	NULL	NULL	0	NULL	previously established rules	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A new hierarchical key for the identification of triacyl quinic acids is presented , based on previously established rules of fragmentation .
	manualset3
132198	5	406642	5	NULL	NULL	0	NULL	fragmentation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A new hierarchical key for the identification of triacyl quinic acids is presented , based on previously established rules of fragmentation .
	manualset3
132199	1	406643	5	NULL	NULL	0	NULL	mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Searching for the mechanism underlying the anti-TNF-alpha effect of NIM , it was found that the drug reduced nuclear factor kappa B activation through diminished nuclear levels of p-65 accompanied by a protective effect against the cardiovascular alterations and mortality seen during endotoxemia .
	manualset3
132200	2	406643	5	NULL	NULL	0	NULL	anti-TNF-alpha effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Searching for the mechanism underlying the anti-TNF-alpha effect of NIM , it was found that the drug reduced nuclear factor kappa B activation through diminished nuclear levels of p-65 accompanied by a protective effect against the cardiovascular alterations and mortality seen during endotoxemia .
	manualset3
132201	3	406643	5	NULL	NULL	0	NULL	NIM	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Searching for the mechanism underlying the anti-TNF-alpha effect of NIM , it was found that the drug reduced nuclear factor kappa B activation through diminished nuclear levels of p-65 accompanied by a protective effect against the cardiovascular alterations and mortality seen during endotoxemia .
	manualset3
132202	4	406643	5	NULL	NULL	0	NULL	drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Searching for the mechanism underlying the anti-TNF-alpha effect of NIM , it was found that the drug reduced nuclear factor kappa B activation through diminished nuclear levels of p-65 accompanied by a protective effect against the cardiovascular alterations and mortality seen during endotoxemia .
	manualset3
132203	5	406643	5	NULL	NULL	0	NULL	nuclear factor kappa B activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Searching for the mechanism underlying the anti-TNF-alpha effect of NIM , it was found that the drug reduced nuclear factor kappa B activation through diminished nuclear levels of p-65 accompanied by a protective effect against the cardiovascular alterations and mortality seen during endotoxemia .
	manualset3
132204	6	406643	5	NULL	NULL	0	NULL	diminished nuclear levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Searching for the mechanism underlying the anti-TNF-alpha effect of NIM , it was found that the drug reduced nuclear factor kappa B activation through diminished nuclear levels of p-65 accompanied by a protective effect against the cardiovascular alterations and mortality seen during endotoxemia .
	manualset3
132205	7	406643	5	NULL	NULL	0	NULL	p-65	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Searching for the mechanism underlying the anti-TNF-alpha effect of NIM , it was found that the drug reduced nuclear factor kappa B activation through diminished nuclear levels of p-65 accompanied by a protective effect against the cardiovascular alterations and mortality seen during endotoxemia .
	manualset3
132206	8	406643	5	NULL	NULL	0	NULL	protective effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Searching for the mechanism underlying the anti-TNF-alpha effect of NIM , it was found that the drug reduced nuclear factor kappa B activation through diminished nuclear levels of p-65 accompanied by a protective effect against the cardiovascular alterations and mortality seen during endotoxemia .
	manualset3
132207	9	406643	5	NULL	NULL	0	NULL	cardiovascular alterations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Searching for the mechanism underlying the anti-TNF-alpha effect of NIM , it was found that the drug reduced nuclear factor kappa B activation through diminished nuclear levels of p-65 accompanied by a protective effect against the cardiovascular alterations and mortality seen during endotoxemia .
	manualset3
132208	10	406643	5	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Searching for the mechanism underlying the anti-TNF-alpha effect of NIM , it was found that the drug reduced nuclear factor kappa B activation through diminished nuclear levels of p-65 accompanied by a protective effect against the cardiovascular alterations and mortality seen during endotoxemia .
	manualset3
132209	11	406643	5	NULL	NULL	0	NULL	endotoxemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Searching for the mechanism underlying the anti-TNF-alpha effect of NIM , it was found that the drug reduced nuclear factor kappa B activation through diminished nuclear levels of p-65 accompanied by a protective effect against the cardiovascular alterations and mortality seen during endotoxemia .
	manualset3
132210	1	406644	5	NULL	NULL	NULL	NULL	Seasonal variations	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Seasonal variations in serum protein bound iodine on civilian Japanese and Caucasians in Japan .
	manualset3
132211	2	406644	5	NULL	NULL	0	NULL	serum protein bound iodine	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Seasonal variations in serum protein bound iodine on civilian Japanese and Caucasians in Japan .
	manualset3
132212	3	406644	5	NULL	NULL	0	NULL	civilian Japanese	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Seasonal variations in serum protein bound iodine on civilian Japanese and Caucasians in Japan .
	manualset3
132213	4	406644	5	NULL	NULL	0	NULL	Caucasians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Seasonal variations in serum protein bound iodine on civilian Japanese and Caucasians in Japan .
	manualset3
132214	5	406644	5	NULL	NULL	0	NULL	Japan	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Seasonal variations in serum protein bound iodine on civilian Japanese and Caucasians in Japan .
	manualset3
132215	1	406645	5	NULL	NULL	0	NULL	Seasonal variations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Seasonal variations of lithium plasma levels .
	manualset3
132216	2	406645	5	NULL	NULL	0	NULL	lithium plasma levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Seasonal variations of lithium plasma levels .
	manualset3
132217	1	406646	5	NULL	NULL	0	NULL	Seasonality	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Seasonality overrides the effects of other farmworker characteristics in predicting detection of pesticide urinary metabolites .
	manualset3
132218	2	406646	5	NULL	NULL	0	NULL	farmworker characteristics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Seasonality overrides the effects of other farmworker characteristics in predicting detection of pesticide urinary metabolites .
	manualset3
132219	3	406646	5	NULL	NULL	0	NULL	detection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Seasonality overrides the effects of other farmworker characteristics in predicting detection of pesticide urinary metabolites .
	manualset3
132220	4	406646	5	NULL	NULL	0	NULL	pesticide urinary metabolites	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Seasonality overrides the effects of other farmworker characteristics in predicting detection of pesticide urinary metabolites .
	manualset3
134864	5	406646	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Seasonality overrides the effects of other farmworker characteristics in predicting detection of pesticide urinary metabolites .
	manualset3
132221	1	406647	5	NULL	NULL	0	NULL	constitutive properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Seat constitutive properties such as stiffness and energy absorption were not significantly correlated with occupant head-neck kinematics .
	manualset3
132222	2	406647	5	NULL	NULL	0	NULL	stiffness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Seat constitutive properties such as stiffness and energy absorption were not significantly correlated with occupant head-neck kinematics .
	manualset3
132223	3	406647	5	NULL	NULL	0	NULL	energy absorption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Seat constitutive properties such as stiffness and energy absorption were not significantly correlated with occupant head-neck kinematics .
	manualset3
132224	4	406647	5	NULL	NULL	0	NULL	occupant head-neck kinematics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Seat constitutive properties such as stiffness and energy absorption were not significantly correlated with occupant head-neck kinematics .
	manualset3
132225	1	406648	5	NULL	NULL	0	NULL	Seborrheic dermatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Seborrheic dermatitis ; supplemental treatment with vitamin B12 .
	manualset3
132226	2	406648	5	NULL	NULL	0	NULL	supplemental treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Seborrheic dermatitis ; supplemental treatment with vitamin B12 .
	manualset3
132227	3	406648	5	NULL	NULL	0	NULL	vitamin B12	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Seborrheic dermatitis ; supplemental treatment with vitamin B12 .
	manualset3
132228	1	406649	5	NULL	NULL	0	NULL	Second-hand Smoke	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Second-hand Smoke : A neglected public health challenge .
	manualset3
132229	2	406649	5	NULL	NULL	0	NULL	public health challenge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Second-hand Smoke : A neglected public health challenge .
	manualset3
132230	1	406650	5	NULL	NULL	0	NULL	n3-PUFA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Second generation n3-PUFA depleted female rats is a good animal model for metabolic syndrome as it displays characteristic features such as liver steatosis , visceral obesity , and insulin resistance .
	manualset3
132231	2	406650	5	NULL	NULL	0	NULL	female rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Second generation n3-PUFA depleted female rats is a good animal model for metabolic syndrome as it displays characteristic features such as liver steatosis , visceral obesity , and insulin resistance .
	manualset3
132232	3	406650	5	NULL	NULL	0	NULL	good animal model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Second generation n3-PUFA depleted female rats is a good animal model for metabolic syndrome as it displays characteristic features such as liver steatosis , visceral obesity , and insulin resistance .
	manualset3
132233	4	406650	5	NULL	NULL	0	NULL	metabolic syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Second generation n3-PUFA depleted female rats is a good animal model for metabolic syndrome as it displays characteristic features such as liver steatosis , visceral obesity , and insulin resistance .
	manualset3
132234	5	406650	5	NULL	NULL	0	NULL	characteristic features	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Second generation n3-PUFA depleted female rats is a good animal model for metabolic syndrome as it displays characteristic features such as liver steatosis , visceral obesity , and insulin resistance .
	manualset3
132235	6	406650	5	NULL	NULL	0	NULL	liver steatosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Second generation n3-PUFA depleted female rats is a good animal model for metabolic syndrome as it displays characteristic features such as liver steatosis , visceral obesity , and insulin resistance .
	manualset3
132236	7	406650	5	NULL	NULL	0	NULL	visceral obesity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Second generation n3-PUFA depleted female rats is a good animal model for metabolic syndrome as it displays characteristic features such as liver steatosis , visceral obesity , and insulin resistance .
	manualset3
132237	8	406650	5	NULL	NULL	0	NULL	 insulin resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Second generation n3-PUFA depleted female rats is a good animal model for metabolic syndrome as it displays characteristic features such as liver steatosis , visceral obesity , and insulin resistance .
	manualset3
132259	1	406651	5	NULL	NULL	0	NULL	procoagulant environment	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Second , a procoagulant environment may promote cancer in different ways .
	manualset3
132260	2	406651	5	NULL	NULL	0	NULL	cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Second , a procoagulant environment may promote cancer in different ways .
	manualset3
132261	1	406652	5	NULL	NULL	0	NULL	kynurenine metabolites	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Second , kynurenine metabolites such as 3-hydroxy-kynurenine ( 3-OH-KYN ) and quinolinic acid ( QUIN ) have toxic effects on brain function .
	manualset3
132262	2	406652	5	NULL	NULL	0	NULL	3-hydroxy-kynurenine ( 3-OH-KYN )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Second , kynurenine metabolites such as 3-hydroxy-kynurenine ( 3-OH-KYN ) and quinolinic acid ( QUIN ) have toxic effects on brain function .
	manualset3
132263	3	406652	5	NULL	NULL	0	NULL	quinolinic acid ( QUIN )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Second , kynurenine metabolites such as 3-hydroxy-kynurenine ( 3-OH-KYN ) and quinolinic acid ( QUIN ) have toxic effects on brain function .
	manualset3
132264	4	406652	5	NULL	NULL	0	NULL	toxic effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Second , kynurenine metabolites such as 3-hydroxy-kynurenine ( 3-OH-KYN ) and quinolinic acid ( QUIN ) have toxic effects on brain function .
	manualset3
132265	5	406652	5	NULL	NULL	0	NULL	brain function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Second , kynurenine metabolites such as 3-hydroxy-kynurenine ( 3-OH-KYN ) and quinolinic acid ( QUIN ) have toxic effects on brain function .
	manualset3
132266	1	406653	5	NULL	NULL	NULL	NULL	body of research 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Second , there is a large and consistent body of research demonstrating that emotion regulation strategies can modulate emotional responding , and this finding is observed in both behavioral and neuroimaging studies .
	manualset3
132267	2	406653	5	NULL	NULL	0	NULL	emotion regulation strategies	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Second , there is a large and consistent body of research demonstrating that emotion regulation strategies can modulate emotional responding , and this finding is observed in both behavioral and neuroimaging studies .
	manualset3
132268	3	406653	5	NULL	NULL	0	NULL	emotional responding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Second , there is a large and consistent body of research demonstrating that emotion regulation strategies can modulate emotional responding , and this finding is observed in both behavioral and neuroimaging studies .
	manualset3
132269	4	406653	5	NULL	NULL	0	NULL	behavioral studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Second , there is a large and consistent body of research demonstrating that emotion regulation strategies can modulate emotional responding , and this finding is observed in both behavioral and neuroimaging studies .
	manualset3
132270	5	406653	5	NULL	NULL	0	NULL	neuroimaging studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Second , there is a large and consistent body of research demonstrating that emotion regulation strategies can modulate emotional responding , and this finding is observed in both behavioral and neuroimaging studies .
	manualset3
134865	6	406653	5	NULL	NULL	0	NULL	finding 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Second , there is a large and consistent body of research demonstrating that emotion regulation strategies can modulate emotional responding , and this finding is observed in both behavioral and neuroimaging studies .
	manualset3
132271	1	406654	5	NULL	NULL	0	NULL	diabetic rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Second , we switched diabetic rats from high-carbohydrate diet to high-fat diet , without choice .
	manualset3
132272	2	406654	5	NULL	NULL	0	NULL	high-carbohydrate diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Second , we switched diabetic rats from high-carbohydrate diet to high-fat diet , without choice .
	manualset3
132273	3	406654	5	NULL	NULL	0	NULL	high-fat diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Second , we switched diabetic rats from high-carbohydrate diet to high-fat diet , without choice .
	manualset3
134867	4	406654	5	NULL	NULL	0	NULL	choice 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Second , we switched diabetic rats from high-carbohydrate diet to high-fat diet , without choice .
	manualset3
132274	1	406655	5	NULL	NULL	0	NULL	Secondary liver involvement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Secondary liver involvement during Hodgkin 's and non-Hodgkin 's lymphoma is frequent .
	manualset3
132275	2	406655	5	NULL	NULL	0	NULL	Hodgkin 's lymphoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Secondary liver involvement during Hodgkin 's and non-Hodgkin 's lymphoma is frequent .
	manualset3
132276	3	406655	5	NULL	NULL	0	NULL	non-Hodgkin 's lymphoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Secondary liver involvement during Hodgkin 's and non-Hodgkin 's lymphoma is frequent .
	manualset3
132277	1	406656	5	NULL	NULL	0	NULL	Secondary radiation doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Secondary radiation doses of intensity-modulated radiotherapy and proton beam therapy in patients with lung and liver cancer .
	manualset3
132278	2	406656	5	NULL	NULL	0	NULL	intensity-modulated radiotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Secondary radiation doses of intensity-modulated radiotherapy and proton beam therapy in patients with lung and liver cancer .
	manualset3
132279	3	406656	5	NULL	NULL	0	NULL	proton beam therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Secondary radiation doses of intensity-modulated radiotherapy and proton beam therapy in patients with lung and liver cancer .
	manualset3
132280	4	406656	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Secondary radiation doses of intensity-modulated radiotherapy and proton beam therapy in patients with lung and liver cancer .
	manualset3
132281	5	406656	5	NULL	NULL	0	NULL	lung cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Secondary radiation doses of intensity-modulated radiotherapy and proton beam therapy in patients with lung and liver cancer .
	manualset3
132282	6	406656	5	NULL	NULL	0	NULL	liver cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Secondary radiation doses of intensity-modulated radiotherapy and proton beam therapy in patients with lung and liver cancer .
	manualset3
132283	1	406657	5	NULL	NULL	0	NULL	Secondary structure predictions	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Secondary structure predictions and molecular modelling suggested that Spi would adopt a structure similar to the SpeB propeptide .
	manualset3
132284	2	406657	5	NULL	NULL	0	NULL	molecular modelling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Secondary structure predictions and molecular modelling suggested that Spi would adopt a structure similar to the SpeB propeptide .
	manualset3
132285	3	406657	5	NULL	NULL	0	NULL	Spi	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Secondary structure predictions and molecular modelling suggested that Spi would adopt a structure similar to the SpeB propeptide .
	manualset3
132286	4	406657	5	NULL	NULL	0	NULL	structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Secondary structure predictions and molecular modelling suggested that Spi would adopt a structure similar to the SpeB propeptide .
	manualset3
132287	5	406657	5	NULL	NULL	0	NULL	SpeB propeptide	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Secondary structure predictions and molecular modelling suggested that Spi would adopt a structure similar to the SpeB propeptide .
	manualset3
132288	1	406658	5	NULL	NULL	0	NULL	charge alignment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Secondly , the charge alignment in the Asp-102 / His-57 / tetrahedral intermediate system implies that the curvature of the potential surface along the conformational coordinates in this state is much lower than in the initial enzyme-substrate and final acyl states .
	manualset3
132289	2	406658	5	NULL	NULL	NULL	NULL	Asp-102 / His-57 / tetrahedral intermediate system	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Secondly , the charge alignment in the Asp-102 / His-57 / tetrahedral intermediate system implies that the curvature of the potential surface along the conformational coordinates in this state is much lower than in the initial enzyme-substrate and final acyl states .
	manualset3
132290	3	406658	5	NULL	NULL	0	NULL	curvature	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Secondly , the charge alignment in the Asp-102 / His-57 / tetrahedral intermediate system implies that the curvature of the potential surface along the conformational coordinates in this state is much lower than in the initial enzyme-substrate and final acyl states .
	manualset3
132291	4	406658	5	NULL	NULL	0	NULL	potential surface	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Secondly , the charge alignment in the Asp-102 / His-57 / tetrahedral intermediate system implies that the curvature of the potential surface along the conformational coordinates in this state is much lower than in the initial enzyme-substrate and final acyl states .
	manualset3
132292	5	406658	5	NULL	NULL	0	NULL	conformational coordinates	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Secondly , the charge alignment in the Asp-102 / His-57 / tetrahedral intermediate system implies that the curvature of the potential surface along the conformational coordinates in this state is much lower than in the initial enzyme-substrate and final acyl states .
	manualset3
132293	6	406658	5	NULL	NULL	0	NULL	state	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Secondly , the charge alignment in the Asp-102 / His-57 / tetrahedral intermediate system implies that the curvature of the potential surface along the conformational coordinates in this state is much lower than in the initial enzyme-substrate and final acyl states .
	manualset3
132294	7	406658	5	NULL	NULL	0	NULL	initial enzyme-substrate	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Secondly , the charge alignment in the Asp-102 / His-57 / tetrahedral intermediate system implies that the curvature of the potential surface along the conformational coordinates in this state is much lower than in the initial enzyme-substrate and final acyl states .
	manualset3
132295	8	406658	5	NULL	NULL	0	NULL	final acyl states	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Secondly , the charge alignment in the Asp-102 / His-57 / tetrahedral intermediate system implies that the curvature of the potential surface along the conformational coordinates in this state is much lower than in the initial enzyme-substrate and final acyl states .
	manualset3
132296	1	406659	5	NULL	NULL	0	NULL	Secreted proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Secreted and transmembrane proteins are critical to the cell-cell interactions governing normal development and carcinogenesis .
	manualset3
132297	2	406659	5	NULL	NULL	0	NULL	transmembrane proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Secreted and transmembrane proteins are critical to the cell-cell interactions governing normal development and carcinogenesis .
	manualset3
132298	3	406659	5	NULL	NULL	0	NULL	cell-cell interactions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Secreted and transmembrane proteins are critical to the cell-cell interactions governing normal development and carcinogenesis .
	manualset3
132299	4	406659	5	NULL	NULL	0	NULL	normal development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Secreted and transmembrane proteins are critical to the cell-cell interactions governing normal development and carcinogenesis .
	manualset3
132300	5	406659	5	NULL	NULL	0	NULL	carcinogenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Secreted and transmembrane proteins are critical to the cell-cell interactions governing normal development and carcinogenesis .
	manualset3
132301	1	406660	5	NULL	NULL	0	NULL	Section 1	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Section 1 : acute coronary syndromes ( acute myocardial infarction ) .
	manualset3
132302	2	406660	5	NULL	NULL	0	NULL	acute coronary syndromes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Section 1 : acute coronary syndromes ( acute myocardial infarction ) .
	manualset3
132303	3	406660	5	NULL	NULL	NULL	NULL	acute myocardial infarction	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Section 1 : acute coronary syndromes ( acute myocardial infarction ) .
	manualset3
132590	1	406661	5	NULL	NULL	0	NULL	Sections 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sections were incubated with rabbit polyclonal antiserum against the catalytic part of the TrkB receptor , thus only binding to full-length TrkB receptors , and examined by immunofluorescence microscopy and EM immunocytochemistry .
	manualset3
132591	2	406661	5	NULL	NULL	0	NULL	rabbit polyclonal antiserum	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Sections were incubated with rabbit polyclonal antiserum against the catalytic part of the TrkB receptor , thus only binding to full-length TrkB receptors , and examined by immunofluorescence microscopy and EM immunocytochemistry .
	manualset3
132592	3	406661	5	NULL	NULL	0	NULL	catalytic part	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sections were incubated with rabbit polyclonal antiserum against the catalytic part of the TrkB receptor , thus only binding to full-length TrkB receptors , and examined by immunofluorescence microscopy and EM immunocytochemistry .
	manualset3
132593	4	406661	5	NULL	NULL	0	NULL	TrkB receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sections were incubated with rabbit polyclonal antiserum against the catalytic part of the TrkB receptor , thus only binding to full-length TrkB receptors , and examined by immunofluorescence microscopy and EM immunocytochemistry .
	manualset3
132594	5	406661	5	NULL	NULL	0	NULL	full-length TrkB receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sections were incubated with rabbit polyclonal antiserum against the catalytic part of the TrkB receptor , thus only binding to full-length TrkB receptors , and examined by immunofluorescence microscopy and EM immunocytochemistry .
	manualset3
132595	6	406661	5	NULL	NULL	0	NULL	immunofluorescence microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sections were incubated with rabbit polyclonal antiserum against the catalytic part of the TrkB receptor , thus only binding to full-length TrkB receptors , and examined by immunofluorescence microscopy and EM immunocytochemistry .
	manualset3
132596	7	406661	5	NULL	NULL	0	NULL	EM immunocytochemistry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sections were incubated with rabbit polyclonal antiserum against the catalytic part of the TrkB receptor , thus only binding to full-length TrkB receptors , and examined by immunofluorescence microscopy and EM immunocytochemistry .
	manualset3
132597	1	406662	5	NULL	NULL	0	NULL	Security 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Security : melding lessons of the past with trends of the future .
	manualset3
132598	2	406662	5	NULL	NULL	0	NULL	past 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Security : melding lessons of the past with trends of the future .
	manualset3
132599	3	406662	5	NULL	NULL	0	NULL	future 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Security : melding lessons of the past with trends of the future .
	manualset3
134869	4	406662	5	NULL	NULL	0	NULL	lessons 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Security : melding lessons of the past with trends of the future .
	manualset3
134870	5	406662	5	NULL	NULL	0	NULL	trends 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Security : melding lessons of the past with trends of the future .
	manualset3
132600	1	406663	5	NULL	NULL	0	NULL	Case 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( Case of intravascular lymphoma diagnosed by transbronchial lung biopsy , with transient spontaneous remission ) .
	manualset3
132601	2	406663	5	NULL	NULL	0	NULL	intravascular lymphoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Case of intravascular lymphoma diagnosed by transbronchial lung biopsy , with transient spontaneous remission ) .
	manualset3
132602	3	406663	5	NULL	NULL	0	NULL	transbronchial lung biopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Case of intravascular lymphoma diagnosed by transbronchial lung biopsy , with transient spontaneous remission ) .
	manualset3
132603	4	406663	5	NULL	NULL	0	NULL	transient spontaneous remission	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Case of intravascular lymphoma diagnosed by transbronchial lung biopsy , with transient spontaneous remission ) .
	manualset3
132604	1	406664	5	NULL	NULL	0	NULL	Sedation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Sedation of children for CT and MRI scanning .
	manualset3
132605	2	406664	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sedation of children for CT and MRI scanning .
	manualset3
132606	3	406664	5	NULL	NULL	0	NULL	CT scanning 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Sedation of children for CT and MRI scanning .
	manualset3
132607	4	406664	5	NULL	NULL	0	NULL	MRI scanning 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Sedation of children for CT and MRI scanning .
	manualset3
132608	1	406665	5	NULL	NULL	0	NULL	Sedimentation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sedimentation and actinomycin D binding studies of partially denatured crab dAT .
	manualset3
132609	2	406665	5	NULL	NULL	0	NULL	actinomycin D binding studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sedimentation and actinomycin D binding studies of partially denatured crab dAT .
	manualset3
132610	3	406665	5	NULL	NULL	0	NULL	partially denatured crab dAT	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Sedimentation and actinomycin D binding studies of partially denatured crab dAT .
	manualset3
132611	1	406666	5	NULL	NULL	NULL	NULL	Sedimentation equilibrium and velocity experiments	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Sedimentation equilibrium and velocity experiments demonstrated that , after removal of the interchain disulfide bond , GDNF remains as a non-covalent dimer and is stable at pH 7.0 .
	manualset3
132612	2	406666	5	NULL	NULL	0	NULL	interchain disulfide bond	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sedimentation equilibrium and velocity experiments demonstrated that , after removal of the interchain disulfide bond , GDNF remains as a non-covalent dimer and is stable at pH 7.0 .
	manualset3
132613	3	406666	5	NULL	NULL	0	NULL	GDNF 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sedimentation equilibrium and velocity experiments demonstrated that , after removal of the interchain disulfide bond , GDNF remains as a non-covalent dimer and is stable at pH 7.0 .
	manualset3
132614	4	406666	5	NULL	NULL	0	NULL	non-covalent dimer 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sedimentation equilibrium and velocity experiments demonstrated that , after removal of the interchain disulfide bond , GDNF remains as a non-covalent dimer and is stable at pH 7.0 .
	manualset3
132615	5	406666	5	NULL	NULL	0	NULL	pH 7.0	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sedimentation equilibrium and velocity experiments demonstrated that , after removal of the interchain disulfide bond , GDNF remains as a non-covalent dimer and is stable at pH 7.0 .
	manualset3
134871	6	406666	5	NULL	NULL	0	NULL	removal 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sedimentation equilibrium and velocity experiments demonstrated that , after removal of the interchain disulfide bond , GDNF remains as a non-covalent dimer and is stable at pH 7.0 .
	manualset3
132616	1	406667	5	NULL	NULL	0	NULL	Commentary 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	See accompanying Commentary by Jin and Cate DOI : 10.1002 / biot .201100489 .
	manualset3
132617	2	406667	5	NULL	NULL	0	NULL	Jin	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	See accompanying Commentary by Jin and Cate DOI : 10.1002 / biot .201100489 .
	manualset3
132618	3	406667	5	NULL	NULL	0	NULL	Cate 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	See accompanying Commentary by Jin and Cate DOI : 10.1002 / biot .201100489 .
	manualset3
132619	4	406667	5	NULL	NULL	0	NULL	DOI : 10.1002 / biot .201100489	Citation												NULL		0	NULL	NULL	NULL	NULL	NULL	See accompanying Commentary by Jin and Cate DOI : 10.1002 / biot .201100489 .
	manualset3
132620	1	406668	5	NULL	NULL	0	NULL	Seed-mediated growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Seed-mediated growth of gold nanoparticles on glassy carbon ( GC ) surfaces was developed .
	manualset3
132621	2	406668	5	NULL	NULL	NULL	NULL	gold nanoparticles	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Seed-mediated growth of gold nanoparticles on glassy carbon ( GC ) surfaces was developed .
	manualset3
132622	3	406668	5	NULL	NULL	0	NULL	glassy carbon ( GC ) surfaces	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Seed-mediated growth of gold nanoparticles on glassy carbon ( GC ) surfaces was developed .
	manualset3
132623	1	406669	5	NULL	NULL	0	NULL	Seeds 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Seeds from transgenic Arabidopsis thaliana plants expressing the Escherichia coli uidA gene encoding beta-glucuronidase ( GUS ) under the control of the AOS promoter were mutagenized with ethylmethane sulfonate and the progeny was screened for individuals exhibiting constitutive expression of uidA in the absence of an added octadecanoid .
	manualset3
132624	2	406669	5	NULL	NULL	0	NULL	transgenic Arabidopsis thaliana plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Seeds from transgenic Arabidopsis thaliana plants expressing the Escherichia coli uidA gene encoding beta-glucuronidase ( GUS ) under the control of the AOS promoter were mutagenized with ethylmethane sulfonate and the progeny was screened for individuals exhibiting constitutive expression of uidA in the absence of an added octadecanoid .
	manualset3
132625	3	406669	5	NULL	NULL	0	NULL	Escherichia coli uidA gene encoding beta-glucuronidase ( GUS ) 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Seeds from transgenic Arabidopsis thaliana plants expressing the Escherichia coli uidA gene encoding beta-glucuronidase ( GUS ) under the control of the AOS promoter were mutagenized with ethylmethane sulfonate and the progeny was screened for individuals exhibiting constitutive expression of uidA in the absence of an added octadecanoid .
	manualset3
132626	4	406669	5	NULL	NULL	0	NULL	AOS promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Seeds from transgenic Arabidopsis thaliana plants expressing the Escherichia coli uidA gene encoding beta-glucuronidase ( GUS ) under the control of the AOS promoter were mutagenized with ethylmethane sulfonate and the progeny was screened for individuals exhibiting constitutive expression of uidA in the absence of an added octadecanoid .
	manualset3
132627	5	406669	5	NULL	NULL	0	NULL	ethylmethane sulfonate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Seeds from transgenic Arabidopsis thaliana plants expressing the Escherichia coli uidA gene encoding beta-glucuronidase ( GUS ) under the control of the AOS promoter were mutagenized with ethylmethane sulfonate and the progeny was screened for individuals exhibiting constitutive expression of uidA in the absence of an added octadecanoid .
	manualset3
132628	6	406669	5	NULL	NULL	0	NULL	progeny 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Seeds from transgenic Arabidopsis thaliana plants expressing the Escherichia coli uidA gene encoding beta-glucuronidase ( GUS ) under the control of the AOS promoter were mutagenized with ethylmethane sulfonate and the progeny was screened for individuals exhibiting constitutive expression of uidA in the absence of an added octadecanoid .
	manualset3
132629	7	406669	5	NULL	NULL	0	NULL	individuals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Seeds from transgenic Arabidopsis thaliana plants expressing the Escherichia coli uidA gene encoding beta-glucuronidase ( GUS ) under the control of the AOS promoter were mutagenized with ethylmethane sulfonate and the progeny was screened for individuals exhibiting constitutive expression of uidA in the absence of an added octadecanoid .
	manualset3
132630	8	406669	5	NULL	NULL	0	NULL	constitutive expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Seeds from transgenic Arabidopsis thaliana plants expressing the Escherichia coli uidA gene encoding beta-glucuronidase ( GUS ) under the control of the AOS promoter were mutagenized with ethylmethane sulfonate and the progeny was screened for individuals exhibiting constitutive expression of uidA in the absence of an added octadecanoid .
	manualset3
132631	9	406669	5	NULL	NULL	0	NULL	uidA 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Seeds from transgenic Arabidopsis thaliana plants expressing the Escherichia coli uidA gene encoding beta-glucuronidase ( GUS ) under the control of the AOS promoter were mutagenized with ethylmethane sulfonate and the progeny was screened for individuals exhibiting constitutive expression of uidA in the absence of an added octadecanoid .
	manualset3
132632	10	406669	5	NULL	NULL	0	NULL	absence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Seeds from transgenic Arabidopsis thaliana plants expressing the Escherichia coli uidA gene encoding beta-glucuronidase ( GUS ) under the control of the AOS promoter were mutagenized with ethylmethane sulfonate and the progeny was screened for individuals exhibiting constitutive expression of uidA in the absence of an added octadecanoid .
	manualset3
132633	11	406669	5	NULL	NULL	0	NULL	octadecanoid 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Seeds from transgenic Arabidopsis thaliana plants expressing the Escherichia coli uidA gene encoding beta-glucuronidase ( GUS ) under the control of the AOS promoter were mutagenized with ethylmethane sulfonate and the progeny was screened for individuals exhibiting constitutive expression of uidA in the absence of an added octadecanoid .
	manualset3
134873	12	406669	5	NULL	NULL	0	NULL	control 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Seeds from transgenic Arabidopsis thaliana plants expressing the Escherichia coli uidA gene encoding beta-glucuronidase ( GUS ) under the control of the AOS promoter were mutagenized with ethylmethane sulfonate and the progeny was screened for individuals exhibiting constitutive expression of uidA in the absence of an added octadecanoid .
	manualset3
132634	1	406670	5	NULL	NULL	NULL	NULL	Segmented polyurethane 	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Segmented polyurethane modified by photopolymerization and cross-linking with 2-methacryloyloxyethyl phosphorylcholine polymer for blood-contacting surfaces of ventricular assist devices .
	manualset3
132635	2	406670	5	NULL	NULL	0	NULL	photopolymerization 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Segmented polyurethane modified by photopolymerization and cross-linking with 2-methacryloyloxyethyl phosphorylcholine polymer for blood-contacting surfaces of ventricular assist devices .
	manualset3
132636	3	406670	5	NULL	NULL	0	NULL	cross-linking	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Segmented polyurethane modified by photopolymerization and cross-linking with 2-methacryloyloxyethyl phosphorylcholine polymer for blood-contacting surfaces of ventricular assist devices .
	manualset3
132637	4	406670	5	NULL	NULL	NULL	NULL	2-methacryloyloxyethyl phosphorylcholine polymer	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Segmented polyurethane modified by photopolymerization and cross-linking with 2-methacryloyloxyethyl phosphorylcholine polymer for blood-contacting surfaces of ventricular assist devices .
	manualset3
132638	5	406670	5	NULL	NULL	0	NULL	blood-contacting surfaces	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Segmented polyurethane modified by photopolymerization and cross-linking with 2-methacryloyloxyethyl phosphorylcholine polymer for blood-contacting surfaces of ventricular assist devices .
	manualset3
132639	6	406670	5	NULL	NULL	0	NULL	ventricular assist devices	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Segmented polyurethane modified by photopolymerization and cross-linking with 2-methacryloyloxyethyl phosphorylcholine polymer for blood-contacting surfaces of ventricular assist devices .
	manualset3
132640	1	406671	5	NULL	NULL	0	NULL	psaE deletion strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Segregated psaE and fpg deletion strains were obtained upon insertional inactivation of both genes in S. elongatus .
	manualset3
132641	2	406671	5	NULL	NULL	0	NULL	fpg deletion strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Segregated psaE and fpg deletion strains were obtained upon insertional inactivation of both genes in S. elongatus .
	manualset3
132642	3	406671	5	NULL	NULL	0	NULL	insertional inactivation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Segregated psaE and fpg deletion strains were obtained upon insertional inactivation of both genes in S. elongatus .
	manualset3
132643	4	406671	5	NULL	NULL	0	NULL	genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Segregated psaE and fpg deletion strains were obtained upon insertional inactivation of both genes in S. elongatus .
	manualset3
132644	5	406671	5	NULL	NULL	0	NULL	S. elongatus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Segregated psaE and fpg deletion strains were obtained upon insertional inactivation of both genes in S. elongatus .
	manualset3
132645	1	406672	5	NULL	NULL	0	NULL	Selected injection sites	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Selected injection sites including saline solution control sites were biopsied at 30 minutes , at 3 , 24 , 48 , and 72 hours , and at 30 days after injection .
	manualset3
132646	2	406672	5	NULL	NULL	0	NULL	saline solution control sites	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Selected injection sites including saline solution control sites were biopsied at 30 minutes , at 3 , 24 , 48 , and 72 hours , and at 30 days after injection .
	manualset3
132647	3	406672	5	NULL	NULL	NULL	NULL	30 minutes	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Selected injection sites including saline solution control sites were biopsied at 30 minutes , at 3 , 24 , 48 , and 72 hours , and at 30 days after injection .
	manualset3
132648	4	406672	5	NULL	NULL	0	NULL	3 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Selected injection sites including saline solution control sites were biopsied at 30 minutes , at 3 , 24 , 48 , and 72 hours , and at 30 days after injection .
	manualset3
132649	5	406672	5	NULL	NULL	0	NULL	24 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Selected injection sites including saline solution control sites were biopsied at 30 minutes , at 3 , 24 , 48 , and 72 hours , and at 30 days after injection .
	manualset3
132650	6	406672	5	NULL	NULL	0	NULL	48 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Selected injection sites including saline solution control sites were biopsied at 30 minutes , at 3 , 24 , 48 , and 72 hours , and at 30 days after injection .
	manualset3
132651	7	406672	5	NULL	NULL	0	NULL	72 hours 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Selected injection sites including saline solution control sites were biopsied at 30 minutes , at 3 , 24 , 48 , and 72 hours , and at 30 days after injection .
	manualset3
132652	8	406672	5	NULL	NULL	0	NULL	30 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Selected injection sites including saline solution control sites were biopsied at 30 minutes , at 3 , 24 , 48 , and 72 hours , and at 30 days after injection .
	manualset3
132653	9	406672	5	NULL	NULL	0	NULL	injection 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Selected injection sites including saline solution control sites were biopsied at 30 minutes , at 3 , 24 , 48 , and 72 hours , and at 30 days after injection .
	manualset3
132654	1	406673	5	NULL	NULL	0	NULL	data sets	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Selecting data sets that include only exposures where tolerably little motion has occurred is an inefficient use of time and flux , especially when detector readout time is significant .
	manualset3
132655	2	406673	5	NULL	NULL	0	NULL	exposures 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Selecting data sets that include only exposures where tolerably little motion has occurred is an inefficient use of time and flux , especially when detector readout time is significant .
	manualset3
132656	3	406673	5	NULL	NULL	0	NULL	motion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Selecting data sets that include only exposures where tolerably little motion has occurred is an inefficient use of time and flux , especially when detector readout time is significant .
	manualset3
132657	4	406673	5	NULL	NULL	0	NULL	inefficient use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Selecting data sets that include only exposures where tolerably little motion has occurred is an inefficient use of time and flux , especially when detector readout time is significant .
	manualset3
132658	5	406673	5	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Selecting data sets that include only exposures where tolerably little motion has occurred is an inefficient use of time and flux , especially when detector readout time is significant .
	manualset3
132659	6	406673	5	NULL	NULL	0	NULL	flux 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Selecting data sets that include only exposures where tolerably little motion has occurred is an inefficient use of time and flux , especially when detector readout time is significant .
	manualset3
132660	7	406673	5	NULL	NULL	0	NULL	detector readout time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Selecting data sets that include only exposures where tolerably little motion has occurred is an inefficient use of time and flux , especially when detector readout time is significant .
	manualset3
132661	1	406674	5	NULL	NULL	0	NULL	Selection 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Selection and design of high-affinity RNA ligands for HIV-1 Rev .
	manualset3
132662	2	406674	5	NULL	NULL	0	NULL	design 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Selection and design of high-affinity RNA ligands for HIV-1 Rev .
	manualset3
132663	3	406674	5	NULL	NULL	0	NULL	high-affinity RNA ligands	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Selection and design of high-affinity RNA ligands for HIV-1 Rev .
	manualset3
132664	4	406674	5	NULL	NULL	0	NULL	HIV-1 Rev	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Selection and design of high-affinity RNA ligands for HIV-1 Rev .
	manualset3
132670	1	406675	5	NULL	NULL	0	NULL	Selection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Selection of an adjuvant for vaccination with the malaria antigen , MSA-2 .
	manualset3
132671	2	406675	5	NULL	NULL	0	NULL	adjuvant 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Selection of an adjuvant for vaccination with the malaria antigen , MSA-2 .
	manualset3
132672	3	406675	5	NULL	NULL	0	NULL	vaccination 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Selection of an adjuvant for vaccination with the malaria antigen , MSA-2 .
	manualset3
132673	4	406675	5	NULL	NULL	0	NULL	malaria antigen , MSA-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Selection of an adjuvant for vaccination with the malaria antigen , MSA-2 .
	manualset3
132765	1	406676	5	NULL	NULL	0	NULL	Selection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Selection of motor assessment tools during the first year of life for infants born preterm will depend on the intended purpose of their use for discrimination , prediction , and/or evaluation .
	manualset3
132766	2	406676	5	NULL	NULL	0	NULL	motor assessment tools 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Selection of motor assessment tools during the first year of life for infants born preterm will depend on the intended purpose of their use for discrimination , prediction , and/or evaluation .
	manualset3
132767	3	406676	5	NULL	NULL	0	NULL	first year	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Selection of motor assessment tools during the first year of life for infants born preterm will depend on the intended purpose of their use for discrimination , prediction , and/or evaluation .
	manualset3
132768	4	406676	5	NULL	NULL	0	NULL	life 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Selection of motor assessment tools during the first year of life for infants born preterm will depend on the intended purpose of their use for discrimination , prediction , and/or evaluation .
	manualset3
132769	5	406676	5	NULL	NULL	0	NULL	infants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Selection of motor assessment tools during the first year of life for infants born preterm will depend on the intended purpose of their use for discrimination , prediction , and/or evaluation .
	manualset3
132839	6	406676	5	NULL	NULL	0	NULL	discrimination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Selection of motor assessment tools during the first year of life for infants born preterm will depend on the intended purpose of their use for discrimination , prediction , and/or evaluation .
	manualset3
132840	7	406676	5	NULL	NULL	0	NULL	prediction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Selection of motor assessment tools during the first year of life for infants born preterm will depend on the intended purpose of their use for discrimination , prediction , and/or evaluation .
	manualset3
132841	8	406676	5	NULL	NULL	0	NULL	evaluation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Selection of motor assessment tools during the first year of life for infants born preterm will depend on the intended purpose of their use for discrimination , prediction , and/or evaluation .
	manualset3
132842	1	406677	5	NULL	NULL	0	NULL	Selective abnormalities 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective abnormalities of prefrontal serotonergic receptors in schizophrenia .
	manualset3
132843	2	406677	5	NULL	NULL	0	NULL	prefrontal serotonergic receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective abnormalities of prefrontal serotonergic receptors in schizophrenia .
	manualset3
132844	3	406677	5	NULL	NULL	0	NULL	schizophrenia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective abnormalities of prefrontal serotonergic receptors in schizophrenia .
	manualset3
132845	1	406678	5	NULL	NULL	0	NULL	Selective attention	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective attention in schizophrenia : relationship to verbal working memory .
	manualset3
132846	2	406678	5	NULL	NULL	0	NULL	schizophrenia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective attention in schizophrenia : relationship to verbal working memory .
	manualset3
132847	3	406678	5	NULL	NULL	0	NULL	relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective attention in schizophrenia : relationship to verbal working memory .
	manualset3
132848	4	406678	5	NULL	NULL	0	NULL	verbal working memory	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective attention in schizophrenia : relationship to verbal working memory .
	manualset3
132849	1	406679	5	NULL	NULL	0	NULL	Selective brushings	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective brushings were conducted for all the respective segmental bronchi in both lungs of 105 patients with positive or suspected positive indications of lung cancer as revealed by sputum cytology .
	manualset3
132850	2	406679	5	NULL	NULL	0	NULL	segmental bronchi	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective brushings were conducted for all the respective segmental bronchi in both lungs of 105 patients with positive or suspected positive indications of lung cancer as revealed by sputum cytology .
	manualset3
132851	3	406679	5	NULL	NULL	0	NULL	lungs 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective brushings were conducted for all the respective segmental bronchi in both lungs of 105 patients with positive or suspected positive indications of lung cancer as revealed by sputum cytology .
	manualset3
132852	4	406679	5	NULL	NULL	0	NULL	105 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective brushings were conducted for all the respective segmental bronchi in both lungs of 105 patients with positive or suspected positive indications of lung cancer as revealed by sputum cytology .
	manualset3
132853	5	406679	5	NULL	NULL	0	NULL	positive or suspected positive indications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective brushings were conducted for all the respective segmental bronchi in both lungs of 105 patients with positive or suspected positive indications of lung cancer as revealed by sputum cytology .
	manualset3
132854	6	406679	5	NULL	NULL	0	NULL	lung cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective brushings were conducted for all the respective segmental bronchi in both lungs of 105 patients with positive or suspected positive indications of lung cancer as revealed by sputum cytology .
	manualset3
132855	7	406679	5	NULL	NULL	0	NULL	sputum cytology	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective brushings were conducted for all the respective segmental bronchi in both lungs of 105 patients with positive or suspected positive indications of lung cancer as revealed by sputum cytology .
	manualset3
132856	1	406680	5	NULL	NULL	0	NULL	Selective defect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective defect in plasmacyoid dendritic cell function in a patient with AIDS-associated atypical genital herpes simplex vegetans treated with imiquimod .
	manualset3
132857	2	406680	5	NULL	NULL	0	NULL	plasmacyoid dendritic cell function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective defect in plasmacyoid dendritic cell function in a patient with AIDS-associated atypical genital herpes simplex vegetans treated with imiquimod .
	manualset3
132858	3	406680	5	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective defect in plasmacyoid dendritic cell function in a patient with AIDS-associated atypical genital herpes simplex vegetans treated with imiquimod .
	manualset3
132859	4	406680	5	NULL	NULL	0	NULL	AIDS-associated atypical genital herpes simplex vegetans	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective defect in plasmacyoid dendritic cell function in a patient with AIDS-associated atypical genital herpes simplex vegetans treated with imiquimod .
	manualset3
132860	5	406680	5	NULL	NULL	0	NULL	imiquimod 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective defect in plasmacyoid dendritic cell function in a patient with AIDS-associated atypical genital herpes simplex vegetans treated with imiquimod .
	manualset3
132861	1	406681	5	NULL	NULL	0	NULL	Selective displacement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective displacement of the binding of ( 3H ) DIP to GT1-1 cells by ( D-Ala2 , N-Me-Phe4 , Gly5-ol ) enkephalin , ( D-Pen2 , D-Pen5 ) enkephalin ( DPDPE ) , and U50488H , which are selective ligands , respectively , for mu - , delta - , and kappa-receptors , was also evaluated .
	manualset3
132862	2	406681	5	NULL	NULL	0	NULL	( 3H ) DIP 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective displacement of the binding of ( 3H ) DIP to GT1-1 cells by ( D-Ala2 , N-Me-Phe4 , Gly5-ol ) enkephalin , ( D-Pen2 , D-Pen5 ) enkephalin ( DPDPE ) , and U50488H , which are selective ligands , respectively , for mu - , delta - , and kappa-receptors , was also evaluated .
	manualset3
132863	3	406681	5	NULL	NULL	0	NULL	GT1-1 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective displacement of the binding of ( 3H ) DIP to GT1-1 cells by ( D-Ala2 , N-Me-Phe4 , Gly5-ol ) enkephalin , ( D-Pen2 , D-Pen5 ) enkephalin ( DPDPE ) , and U50488H , which are selective ligands , respectively , for mu - , delta - , and kappa-receptors , was also evaluated .
	manualset3
132864	4	406681	5	NULL	NULL	0	NULL	( D-Ala2 , N-Me-Phe4 , Gly5-ol ) enkephalin	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective displacement of the binding of ( 3H ) DIP to GT1-1 cells by ( D-Ala2 , N-Me-Phe4 , Gly5-ol ) enkephalin , ( D-Pen2 , D-Pen5 ) enkephalin ( DPDPE ) , and U50488H , which are selective ligands , respectively , for mu - , delta - , and kappa-receptors , was also evaluated .
	manualset3
132865	5	406681	5	NULL	NULL	0	NULL	( D-Pen2 , D-Pen5 ) enkephalin ( DPDPE ) 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective displacement of the binding of ( 3H ) DIP to GT1-1 cells by ( D-Ala2 , N-Me-Phe4 , Gly5-ol ) enkephalin , ( D-Pen2 , D-Pen5 ) enkephalin ( DPDPE ) , and U50488H , which are selective ligands , respectively , for mu - , delta - , and kappa-receptors , was also evaluated .
	manualset3
132866	6	406681	5	NULL	NULL	0	NULL	U50488H 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective displacement of the binding of ( 3H ) DIP to GT1-1 cells by ( D-Ala2 , N-Me-Phe4 , Gly5-ol ) enkephalin , ( D-Pen2 , D-Pen5 ) enkephalin ( DPDPE ) , and U50488H , which are selective ligands , respectively , for mu - , delta - , and kappa-receptors , was also evaluated .
	manualset3
132867	7	406681	5	NULL	NULL	0	NULL	selective ligands 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective displacement of the binding of ( 3H ) DIP to GT1-1 cells by ( D-Ala2 , N-Me-Phe4 , Gly5-ol ) enkephalin , ( D-Pen2 , D-Pen5 ) enkephalin ( DPDPE ) , and U50488H , which are selective ligands , respectively , for mu - , delta - , and kappa-receptors , was also evaluated .
	manualset3
132868	8	406681	5	NULL	NULL	0	NULL	mu - , delta - , and kappa-receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective displacement of the binding of ( 3H ) DIP to GT1-1 cells by ( D-Ala2 , N-Me-Phe4 , Gly5-ol ) enkephalin , ( D-Pen2 , D-Pen5 ) enkephalin ( DPDPE ) , and U50488H , which are selective ligands , respectively , for mu - , delta - , and kappa-receptors , was also evaluated .
	manualset3
132869	1	406682	5	NULL	NULL	0	NULL	Selective expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective expression of S100A7 in lung squamous cell carcinomas and large cell carcinomas but not in adenocarcinomas and small cell carcinomas .
	manualset3
132870	2	406682	5	NULL	NULL	0	NULL	S100A7 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective expression of S100A7 in lung squamous cell carcinomas and large cell carcinomas but not in adenocarcinomas and small cell carcinomas .
	manualset3
132871	3	406682	5	NULL	NULL	0	NULL	lung squamous cell carcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective expression of S100A7 in lung squamous cell carcinomas and large cell carcinomas but not in adenocarcinomas and small cell carcinomas .
	manualset3
132872	4	406682	5	NULL	NULL	0	NULL	large cell carcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective expression of S100A7 in lung squamous cell carcinomas and large cell carcinomas but not in adenocarcinomas and small cell carcinomas .
	manualset3
132873	5	406682	5	NULL	NULL	0	NULL	adenocarcinomas 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective expression of S100A7 in lung squamous cell carcinomas and large cell carcinomas but not in adenocarcinomas and small cell carcinomas .
	manualset3
132874	6	406682	5	NULL	NULL	0	NULL	small cell carcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective expression of S100A7 in lung squamous cell carcinomas and large cell carcinomas but not in adenocarcinomas and small cell carcinomas .
	manualset3
132875	1	406683	5	NULL	NULL	0	NULL	Selective induction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective induction of apoptosis in antigen-presenting cells in mice by Parapoxvirus ovis .
	manualset3
132876	2	406683	5	NULL	NULL	0	NULL	apoptosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective induction of apoptosis in antigen-presenting cells in mice by Parapoxvirus ovis .
	manualset3
132877	3	406683	5	NULL	NULL	0	NULL	antigen-presenting cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective induction of apoptosis in antigen-presenting cells in mice by Parapoxvirus ovis .
	manualset3
132878	4	406683	5	NULL	NULL	0	NULL	mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective induction of apoptosis in antigen-presenting cells in mice by Parapoxvirus ovis .
	manualset3
132879	5	406683	5	NULL	NULL	0	NULL	Parapoxvirus ovis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective induction of apoptosis in antigen-presenting cells in mice by Parapoxvirus ovis .
	manualset3
132880	1	406684	5	NULL	NULL	0	NULL	Selective inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective inhibition of ADAM12 catalytic activity through engineering of tissue inhibitor of metalloproteinase 2 ( TIMP-2 ) .
	manualset3
132881	2	406684	5	NULL	NULL	0	NULL	ADAM12 catalytic activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective inhibition of ADAM12 catalytic activity through engineering of tissue inhibitor of metalloproteinase 2 ( TIMP-2 ) .
	manualset3
132882	3	406684	5	NULL	NULL	0	NULL	tissue inhibitor of metalloproteinase 2 ( TIMP-2 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective inhibition of ADAM12 catalytic activity through engineering of tissue inhibitor of metalloproteinase 2 ( TIMP-2 ) .
	manualset3
134874	4	406684	5	NULL	NULL	0	NULL	engineering 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective inhibition of ADAM12 catalytic activity through engineering of tissue inhibitor of metalloproteinase 2 ( TIMP-2 ) .
	manualset3
132883	1	406685	5	NULL	NULL	0	NULL	Selective inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective inhibition of Pi class GST by the Pi-specific antisera , either at 0 h or at 3 h after initiation of sperm capacitation , leads to a reduction in fertilization rates .
	manualset3
132884	2	406685	5	NULL	NULL	0	NULL	Pi class GST 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective inhibition of Pi class GST by the Pi-specific antisera , either at 0 h or at 3 h after initiation of sperm capacitation , leads to a reduction in fertilization rates .
	manualset3
132885	3	406685	5	NULL	NULL	0	NULL	Pi-specific antisera	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective inhibition of Pi class GST by the Pi-specific antisera , either at 0 h or at 3 h after initiation of sperm capacitation , leads to a reduction in fertilization rates .
	manualset3
132886	4	406685	5	NULL	NULL	0	NULL	 0 h 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective inhibition of Pi class GST by the Pi-specific antisera , either at 0 h or at 3 h after initiation of sperm capacitation , leads to a reduction in fertilization rates .
	manualset3
132887	5	406685	5	NULL	NULL	0	NULL	3 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective inhibition of Pi class GST by the Pi-specific antisera , either at 0 h or at 3 h after initiation of sperm capacitation , leads to a reduction in fertilization rates .
	manualset3
132888	6	406685	5	NULL	NULL	0	NULL	initiation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective inhibition of Pi class GST by the Pi-specific antisera , either at 0 h or at 3 h after initiation of sperm capacitation , leads to a reduction in fertilization rates .
	manualset3
132889	7	406685	5	NULL	NULL	0	NULL	sperm capacitation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective inhibition of Pi class GST by the Pi-specific antisera , either at 0 h or at 3 h after initiation of sperm capacitation , leads to a reduction in fertilization rates .
	manualset3
132890	8	406685	5	NULL	NULL	0	NULL	reduction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective inhibition of Pi class GST by the Pi-specific antisera , either at 0 h or at 3 h after initiation of sperm capacitation , leads to a reduction in fertilization rates .
	manualset3
132891	9	406685	5	NULL	NULL	0	NULL	fertilization rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective inhibition of Pi class GST by the Pi-specific antisera , either at 0 h or at 3 h after initiation of sperm capacitation , leads to a reduction in fertilization rates .
	manualset3
132892	1	406686	5	NULL	NULL	0	NULL	Selenium compounds 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Selenium compounds are known as cancer preventive agents and are also able to ameliorate the toxicity associated with anti-cancer radiation and chemotherapy in mouse models .
	manualset3
132893	2	406686	5	NULL	NULL	0	NULL	cancer preventive agents	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Selenium compounds are known as cancer preventive agents and are also able to ameliorate the toxicity associated with anti-cancer radiation and chemotherapy in mouse models .
	manualset3
132894	3	406686	5	NULL	NULL	0	NULL	toxicity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Selenium compounds are known as cancer preventive agents and are also able to ameliorate the toxicity associated with anti-cancer radiation and chemotherapy in mouse models .
	manualset3
132895	4	406686	5	NULL	NULL	0	NULL	anti-cancer radiation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Selenium compounds are known as cancer preventive agents and are also able to ameliorate the toxicity associated with anti-cancer radiation and chemotherapy in mouse models .
	manualset3
132896	5	406686	5	NULL	NULL	0	NULL	chemotherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Selenium compounds are known as cancer preventive agents and are also able to ameliorate the toxicity associated with anti-cancer radiation and chemotherapy in mouse models .
	manualset3
132897	6	406686	5	NULL	NULL	0	NULL	mouse models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Selenium compounds are known as cancer preventive agents and are also able to ameliorate the toxicity associated with anti-cancer radiation and chemotherapy in mouse models .
	manualset3
132898	1	406687	5	NULL	NULL	0	NULL	Self-Reported and objectively measured physical activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Self-Reported and objectively measured physical activity among a cohort of postpartum women : the PIN Postpartum Study .
	manualset3
132899	2	406687	5	NULL	NULL	0	NULL	cohort	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Self-Reported and objectively measured physical activity among a cohort of postpartum women : the PIN Postpartum Study .
	manualset3
132900	3	406687	5	NULL	NULL	0	NULL	postpartum women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Self-Reported and objectively measured physical activity among a cohort of postpartum women : the PIN Postpartum Study .
	manualset3
132901	4	406687	5	NULL	NULL	0	NULL	PIN Postpartum Study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Self-Reported and objectively measured physical activity among a cohort of postpartum women : the PIN Postpartum Study .
	manualset3
132902	1	406688	5	NULL	NULL	0	NULL	Self-coiling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Self-coiling of Ag2V4O11 nanobelts into perfect nanorings and microloops .
	manualset3
132903	2	406688	5	NULL	NULL	0	NULL	 Ag2V4O11 nanobelts	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Self-coiling of Ag2V4O11 nanobelts into perfect nanorings and microloops .
	manualset3
132904	3	406688	5	NULL	NULL	0	NULL	nanorings 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Self-coiling of Ag2V4O11 nanobelts into perfect nanorings and microloops .
	manualset3
132905	4	406688	5	NULL	NULL	0	NULL	microloops 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Self-coiling of Ag2V4O11 nanobelts into perfect nanorings and microloops .
	manualset3
132906	1	406689	5	NULL	NULL	0	NULL	Self-monitoring	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Self-monitoring of blood glucose in type 2 diabetes and long-term outcome : an epidemiological cohort study .
	manualset3
132907	2	406689	5	NULL	NULL	0	NULL	blood glucose	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Self-monitoring of blood glucose in type 2 diabetes and long-term outcome : an epidemiological cohort study .
	manualset3
132908	3	406689	5	NULL	NULL	0	NULL	type 2 diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Self-monitoring of blood glucose in type 2 diabetes and long-term outcome : an epidemiological cohort study .
	manualset3
132909	4	406689	5	NULL	NULL	0	NULL	 long-term outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Self-monitoring of blood glucose in type 2 diabetes and long-term outcome : an epidemiological cohort study .
	manualset3
132910	5	406689	5	NULL	NULL	0	NULL	epidemiological cohort study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Self-monitoring of blood glucose in type 2 diabetes and long-term outcome : an epidemiological cohort study .
	manualset3
132911	1	406690	5	NULL	NULL	0	NULL	Self-regulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Self-regulation of health behavior : the `` take PRIDE '' program .
	manualset3
132912	2	406690	5	NULL	NULL	0	NULL	health behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Self-regulation of health behavior : the `` take PRIDE '' program .
	manualset3
132913	3	406690	5	NULL	NULL	0	NULL	 `` take PRIDE '' program	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Self-regulation of health behavior : the `` take PRIDE '' program .
	manualset3
132914	1	406691	5	NULL	NULL	0	NULL	Semen samples	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Semen samples with a high percentage of food dye positive , defined as dead , spermatozoa had a low sortability index and ranking .
	manualset3
132915	2	406691	5	NULL	NULL	0	NULL	high percentage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Semen samples with a high percentage of food dye positive , defined as dead , spermatozoa had a low sortability index and ranking .
	manualset3
132916	3	406691	5	NULL	NULL	0	NULL	food dye positive	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Semen samples with a high percentage of food dye positive , defined as dead , spermatozoa had a low sortability index and ranking .
	manualset3
132917	4	406691	5	NULL	NULL	0	NULL	spermatozoa 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Semen samples with a high percentage of food dye positive , defined as dead , spermatozoa had a low sortability index and ranking .
	manualset3
132918	5	406691	5	NULL	NULL	0	NULL	low sortability index	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Semen samples with a high percentage of food dye positive , defined as dead , spermatozoa had a low sortability index and ranking .
	manualset3
134875	6	406691	5	NULL	NULL	0	NULL	ranking 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Semen samples with a high percentage of food dye positive , defined as dead , spermatozoa had a low sortability index and ranking .
	manualset3
132919	1	406692	5	NULL	NULL	0	NULL	Semi-conservative DNA synthesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Semi-conservative DNA synthesis is observed when the isolated , folded E. coli chromosome is supplemented with a DNA-free , soluble enzyme fraction , the four deoxynucleoside 5 ' - triphosphates , ATP , and Mg ( + + ) .
	manualset3
132920	2	406692	5	NULL	NULL	0	NULL	isolated , folded E. coli chromosome	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Semi-conservative DNA synthesis is observed when the isolated , folded E. coli chromosome is supplemented with a DNA-free , soluble enzyme fraction , the four deoxynucleoside 5 ' - triphosphates , ATP , and Mg ( + + ) .
	manualset3
132921	3	406692	5	NULL	NULL	0	NULL	DNA-free , soluble enzyme fraction	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Semi-conservative DNA synthesis is observed when the isolated , folded E. coli chromosome is supplemented with a DNA-free , soluble enzyme fraction , the four deoxynucleoside 5 ' - triphosphates , ATP , and Mg ( + + ) .
	manualset3
132922	4	406692	5	NULL	NULL	0	NULL	four	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Semi-conservative DNA synthesis is observed when the isolated , folded E. coli chromosome is supplemented with a DNA-free , soluble enzyme fraction , the four deoxynucleoside 5 ' - triphosphates , ATP , and Mg ( + + ) .
	manualset3
132923	5	406692	5	NULL	NULL	0	NULL	deoxynucleoside 5 ' - triphosphates	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Semi-conservative DNA synthesis is observed when the isolated , folded E. coli chromosome is supplemented with a DNA-free , soluble enzyme fraction , the four deoxynucleoside 5 ' - triphosphates , ATP , and Mg ( + + ) .
	manualset3
132924	6	406692	5	NULL	NULL	0	NULL	ATP 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Semi-conservative DNA synthesis is observed when the isolated , folded E. coli chromosome is supplemented with a DNA-free , soluble enzyme fraction , the four deoxynucleoside 5 ' - triphosphates , ATP , and Mg ( + + ) .
	manualset3
132925	7	406692	5	NULL	NULL	0	NULL	Mg ( + + )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Semi-conservative DNA synthesis is observed when the isolated , folded E. coli chromosome is supplemented with a DNA-free , soluble enzyme fraction , the four deoxynucleoside 5 ' - triphosphates , ATP , and Mg ( + + ) .
	manualset3
132926	1	406693	5	NULL	NULL	0	NULL	Semi-quantitative RT-PCR results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Semi-quantitative RT-PCR results confirmed that porcine Six1 was highly expressed in skeletal muscle .
	manualset3
132927	2	406693	5	NULL	NULL	0	NULL	porcine Six1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Semi-quantitative RT-PCR results confirmed that porcine Six1 was highly expressed in skeletal muscle .
	manualset3
132928	3	406693	5	NULL	NULL	0	NULL	skeletal muscle	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Semi-quantitative RT-PCR results confirmed that porcine Six1 was highly expressed in skeletal muscle .
	manualset3
132929	1	406694	5	NULL	NULL	0	NULL	Semi-quantitative estimation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Semi-quantitative estimation was performed by using the monoglycoside and diglycoside of quercetin as internal standards .
	manualset3
132930	2	406694	5	NULL	NULL	0	NULL	monoglycoside of quercetin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Semi-quantitative estimation was performed by using the monoglycoside and diglycoside of quercetin as internal standards .
	manualset3
132931	3	406694	5	NULL	NULL	0	NULL	diglycoside of quercetin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Semi-quantitative estimation was performed by using the monoglycoside and diglycoside of quercetin as internal standards .
	manualset3
132932	4	406694	5	NULL	NULL	NULL	NULL	internal standards	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Semi-quantitative estimation was performed by using the monoglycoside and diglycoside of quercetin as internal standards .
	manualset3
132933	1	406695	5	NULL	NULL	0	NULL	Semi-quantitative estimations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Semi-quantitative estimations of nerve densities were made for CGRP-ir and SP-ir fibers innervating the dome , body and base of the urinary bladder .
	manualset3
132934	2	406695	5	NULL	NULL	0	NULL	nerve densities	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Semi-quantitative estimations of nerve densities were made for CGRP-ir and SP-ir fibers innervating the dome , body and base of the urinary bladder .
	manualset3
132935	3	406695	5	NULL	NULL	0	NULL	CGRP-ir fibres	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Semi-quantitative estimations of nerve densities were made for CGRP-ir and SP-ir fibers innervating the dome , body and base of the urinary bladder .
	manualset3
132936	4	406695	5	NULL	NULL	0	NULL	SP-ir fibers	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Semi-quantitative estimations of nerve densities were made for CGRP-ir and SP-ir fibers innervating the dome , body and base of the urinary bladder .
	manualset3
132937	5	406695	5	NULL	NULL	0	NULL	dome of the urinary bladder	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Semi-quantitative estimations of nerve densities were made for CGRP-ir and SP-ir fibers innervating the dome , body and base of the urinary bladder .
	manualset3
132938	6	406695	5	NULL	NULL	0	NULL	body of the urinary bladder	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Semi-quantitative estimations of nerve densities were made for CGRP-ir and SP-ir fibers innervating the dome , body and base of the urinary bladder .
	manualset3
132939	7	406695	5	NULL	NULL	0	NULL	base of the urinary bladder	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Semi-quantitative estimations of nerve densities were made for CGRP-ir and SP-ir fibers innervating the dome , body and base of the urinary bladder .
	manualset3
132940	1	406696	5	NULL	NULL	0	NULL	Semicarbazide-sensitive amine oxidase substrates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Semicarbazide-sensitive amine oxidase substrates fail to induce insulin-like effects in fat cells from AOC3 knockout mice .
	manualset3
132941	2	406696	5	NULL	NULL	0	NULL	insulin-like effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Semicarbazide-sensitive amine oxidase substrates fail to induce insulin-like effects in fat cells from AOC3 knockout mice .
	manualset3
132942	3	406696	5	NULL	NULL	0	NULL	fat cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Semicarbazide-sensitive amine oxidase substrates fail to induce insulin-like effects in fat cells from AOC3 knockout mice .
	manualset3
132943	4	406696	5	NULL	NULL	0	NULL	AOC3 knockout mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Semicarbazide-sensitive amine oxidase substrates fail to induce insulin-like effects in fat cells from AOC3 knockout mice .
	manualset3
132944	1	406697	5	NULL	NULL	0	NULL	Semiconductor quantum dots	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Semiconductor quantum dots are expected to have much slower carrier cooling because the spacing between their discrete electronic levels is much larger than phonon energy .
	manualset3
132945	2	406697	5	NULL	NULL	0	NULL	slower carrier cooling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Semiconductor quantum dots are expected to have much slower carrier cooling because the spacing between their discrete electronic levels is much larger than phonon energy .
	manualset3
132946	3	406697	5	NULL	NULL	0	NULL	 discrete electronic levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Semiconductor quantum dots are expected to have much slower carrier cooling because the spacing between their discrete electronic levels is much larger than phonon energy .
	manualset3
132947	4	406697	5	NULL	NULL	0	NULL	phonon energy 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Semiconductor quantum dots are expected to have much slower carrier cooling because the spacing between their discrete electronic levels is much larger than phonon energy .
	manualset3
132948	1	406698	5	NULL	NULL	0	NULL	Seminal markers	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Seminal markers of epididymal ( neutral alpha-glucosidase ) , prostatic ( prostate specific-antigen and zinc ) , and seminal vesicles function ( fructose ) were measured .
	manualset3
132949	2	406698	5	NULL	NULL	0	NULL	epididymal ( neutral alpha-glucosidase ) function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Seminal markers of epididymal ( neutral alpha-glucosidase ) , prostatic ( prostate specific-antigen and zinc ) , and seminal vesicles function ( fructose ) were measured .
	manualset3
132950	3	406698	5	NULL	NULL	0	NULL	prostatic ( prostate specific-antigen and zinc ) function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Seminal markers of epididymal ( neutral alpha-glucosidase ) , prostatic ( prostate specific-antigen and zinc ) , and seminal vesicles function ( fructose ) were measured .
	manualset3
132951	4	406698	5	NULL	NULL	0	NULL	seminal vesicles function ( fructose )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Seminal markers of epididymal ( neutral alpha-glucosidase ) , prostatic ( prostate specific-antigen and zinc ) , and seminal vesicles function ( fructose ) were measured .
	manualset3
132952	1	406699	5	NULL	NULL	0	NULL	Senescence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Senescence of microvascular endothelial cells is known to play an important role in the pathophysiology of vascular diseases related to ageing , but the accurate mechanism or related genes are not known .
	manualset3
132953	2	406699	5	NULL	NULL	0	NULL	microvascular endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Senescence of microvascular endothelial cells is known to play an important role in the pathophysiology of vascular diseases related to ageing , but the accurate mechanism or related genes are not known .
	manualset3
132954	3	406699	5	NULL	NULL	0	NULL	important role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Senescence of microvascular endothelial cells is known to play an important role in the pathophysiology of vascular diseases related to ageing , but the accurate mechanism or related genes are not known .
	manualset3
132955	4	406699	5	NULL	NULL	NULL	NULL	pathophysiology 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Senescence of microvascular endothelial cells is known to play an important role in the pathophysiology of vascular diseases related to ageing , but the accurate mechanism or related genes are not known .
	manualset3
132956	5	406699	5	NULL	NULL	0	NULL	vascular diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Senescence of microvascular endothelial cells is known to play an important role in the pathophysiology of vascular diseases related to ageing , but the accurate mechanism or related genes are not known .
	manualset3
132957	6	406699	5	NULL	NULL	0	NULL	ageing 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Senescence of microvascular endothelial cells is known to play an important role in the pathophysiology of vascular diseases related to ageing , but the accurate mechanism or related genes are not known .
	manualset3
132958	7	406699	5	NULL	NULL	0	NULL	accurate mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Senescence of microvascular endothelial cells is known to play an important role in the pathophysiology of vascular diseases related to ageing , but the accurate mechanism or related genes are not known .
	manualset3
132959	8	406699	5	NULL	NULL	0	NULL	related genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Senescence of microvascular endothelial cells is known to play an important role in the pathophysiology of vascular diseases related to ageing , but the accurate mechanism or related genes are not known .
	manualset3
132960	1	406700	5	NULL	NULL	0	NULL	Senile plaques ( SPs )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Senile plaques ( SPs ) in CAA cases showed strong ubiquitin positivity but the central amyloid core was negative .
	manualset3
132961	2	406700	5	NULL	NULL	0	NULL	CAA cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Senile plaques ( SPs ) in CAA cases showed strong ubiquitin positivity but the central amyloid core was negative .
	manualset3
132962	3	406700	5	NULL	NULL	0	NULL	strong ubiquitin positivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Senile plaques ( SPs ) in CAA cases showed strong ubiquitin positivity but the central amyloid core was negative .
	manualset3
132963	4	406700	5	NULL	NULL	0	NULL	central amyloid core	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Senile plaques ( SPs ) in CAA cases showed strong ubiquitin positivity but the central amyloid core was negative .
	manualset3
132964	1	406701	5	NULL	NULL	0	NULL	Sense 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sense from nonsense : RNA editing in mitochondria of kinetoplastid protozoa and slime molds .
	manualset3
132965	2	406701	5	NULL	NULL	0	NULL	nonsense 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sense from nonsense : RNA editing in mitochondria of kinetoplastid protozoa and slime molds .
	manualset3
132966	3	406701	5	NULL	NULL	0	NULL	RNA editing	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sense from nonsense : RNA editing in mitochondria of kinetoplastid protozoa and slime molds .
	manualset3
132967	4	406701	5	NULL	NULL	0	NULL	mitochondria 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Sense from nonsense : RNA editing in mitochondria of kinetoplastid protozoa and slime molds .
	manualset3
132968	5	406701	5	NULL	NULL	0	NULL	kinetoplastid protozoa 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sense from nonsense : RNA editing in mitochondria of kinetoplastid protozoa and slime molds .
	manualset3
132969	6	406701	5	NULL	NULL	0	NULL	slime molds	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sense from nonsense : RNA editing in mitochondria of kinetoplastid protozoa and slime molds .
	manualset3
132970	1	406702	5	NULL	NULL	0	NULL	Sensitivity analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitivity analyses elucidate how temperature affects the metabolism and growth of cells through all four stages of fermentation and reveal that there is a qualitative reversal in the factors limiting growth between low and high temperatures .
	manualset3
132971	2	406702	5	NULL	NULL	0	NULL	temperature 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitivity analyses elucidate how temperature affects the metabolism and growth of cells through all four stages of fermentation and reveal that there is a qualitative reversal in the factors limiting growth between low and high temperatures .
	manualset3
132972	3	406702	5	NULL	NULL	0	NULL	metabolism 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitivity analyses elucidate how temperature affects the metabolism and growth of cells through all four stages of fermentation and reveal that there is a qualitative reversal in the factors limiting growth between low and high temperatures .
	manualset3
132973	4	406702	5	NULL	NULL	0	NULL	growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitivity analyses elucidate how temperature affects the metabolism and growth of cells through all four stages of fermentation and reveal that there is a qualitative reversal in the factors limiting growth between low and high temperatures .
	manualset3
132974	5	406702	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitivity analyses elucidate how temperature affects the metabolism and growth of cells through all four stages of fermentation and reveal that there is a qualitative reversal in the factors limiting growth between low and high temperatures .
	manualset3
132975	6	406702	5	NULL	NULL	0	NULL	four stages	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitivity analyses elucidate how temperature affects the metabolism and growth of cells through all four stages of fermentation and reveal that there is a qualitative reversal in the factors limiting growth between low and high temperatures .
	manualset3
132976	7	406702	5	NULL	NULL	0	NULL	fermentation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitivity analyses elucidate how temperature affects the metabolism and growth of cells through all four stages of fermentation and reveal that there is a qualitative reversal in the factors limiting growth between low and high temperatures .
	manualset3
132977	8	406702	5	NULL	NULL	0	NULL	qualitative reversal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitivity analyses elucidate how temperature affects the metabolism and growth of cells through all four stages of fermentation and reveal that there is a qualitative reversal in the factors limiting growth between low and high temperatures .
	manualset3
132978	9	406702	5	NULL	NULL	0	NULL	factors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitivity analyses elucidate how temperature affects the metabolism and growth of cells through all four stages of fermentation and reveal that there is a qualitative reversal in the factors limiting growth between low and high temperatures .
	manualset3
132979	10	406702	5	NULL	NULL	0	NULL	growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitivity analyses elucidate how temperature affects the metabolism and growth of cells through all four stages of fermentation and reveal that there is a qualitative reversal in the factors limiting growth between low and high temperatures .
	manualset3
132980	11	406702	5	NULL	NULL	0	NULL	 low and high temperatures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitivity analyses elucidate how temperature affects the metabolism and growth of cells through all four stages of fermentation and reveal that there is a qualitative reversal in the factors limiting growth between low and high temperatures .
	manualset3
132981	1	406703	5	NULL	NULL	0	NULL	Sensitization 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitization of cells to complement lysis , neutralization of infectious virus and immune precipitation of surface glycoproteins ( region a ) were found to be generally correlated properties of all the antibody preparations analyzed , including antibody prepared specifically against region a antigens .
	manualset3
132982	2	406703	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitization of cells to complement lysis , neutralization of infectious virus and immune precipitation of surface glycoproteins ( region a ) were found to be generally correlated properties of all the antibody preparations analyzed , including antibody prepared specifically against region a antigens .
	manualset3
132983	3	406703	5	NULL	NULL	0	NULL	lysis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitization of cells to complement lysis , neutralization of infectious virus and immune precipitation of surface glycoproteins ( region a ) were found to be generally correlated properties of all the antibody preparations analyzed , including antibody prepared specifically against region a antigens .
	manualset3
132984	4	406703	5	NULL	NULL	0	NULL	neutralization 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitization of cells to complement lysis , neutralization of infectious virus and immune precipitation of surface glycoproteins ( region a ) were found to be generally correlated properties of all the antibody preparations analyzed , including antibody prepared specifically against region a antigens .
	manualset3
132985	5	406703	5	NULL	NULL	0	NULL	infectious virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitization of cells to complement lysis , neutralization of infectious virus and immune precipitation of surface glycoproteins ( region a ) were found to be generally correlated properties of all the antibody preparations analyzed , including antibody prepared specifically against region a antigens .
	manualset3
132986	6	406703	5	NULL	NULL	0	NULL	immune precipitation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitization of cells to complement lysis , neutralization of infectious virus and immune precipitation of surface glycoproteins ( region a ) were found to be generally correlated properties of all the antibody preparations analyzed , including antibody prepared specifically against region a antigens .
	manualset3
132987	7	406703	5	NULL	NULL	0	NULL	surface glycoproteins ( region a ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitization of cells to complement lysis , neutralization of infectious virus and immune precipitation of surface glycoproteins ( region a ) were found to be generally correlated properties of all the antibody preparations analyzed , including antibody prepared specifically against region a antigens .
	manualset3
132988	8	406703	5	NULL	NULL	0	NULL	correlated properties 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitization of cells to complement lysis , neutralization of infectious virus and immune precipitation of surface glycoproteins ( region a ) were found to be generally correlated properties of all the antibody preparations analyzed , including antibody prepared specifically against region a antigens .
	manualset3
132989	9	406703	5	NULL	NULL	0	NULL	antibody preparations	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitization of cells to complement lysis , neutralization of infectious virus and immune precipitation of surface glycoproteins ( region a ) were found to be generally correlated properties of all the antibody preparations analyzed , including antibody prepared specifically against region a antigens .
	manualset3
132990	10	406703	5	NULL	NULL	0	NULL	antibody 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitization of cells to complement lysis , neutralization of infectious virus and immune precipitation of surface glycoproteins ( region a ) were found to be generally correlated properties of all the antibody preparations analyzed , including antibody prepared specifically against region a antigens .
	manualset3
132991	11	406703	5	NULL	NULL	0	NULL	region a antigens	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitization of cells to complement lysis , neutralization of infectious virus and immune precipitation of surface glycoproteins ( region a ) were found to be generally correlated properties of all the antibody preparations analyzed , including antibody prepared specifically against region a antigens .
	manualset3
132992	1	406704	5	NULL	NULL	0	NULL	Sensitized peripheral blood lymphocytes ( PBL )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitized peripheral blood lymphocytes ( PBL ) obtained from canine transmissible venereal sarcoma ( CTVS ) - regressed dogs were more cytotoxic against CTVS cells than non-sensitized PBL from untreated dogs .
	manualset3
132993	2	406704	5	NULL	NULL	0	NULL	canine transmissible venereal sarcoma ( CTVS )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitized peripheral blood lymphocytes ( PBL ) obtained from canine transmissible venereal sarcoma ( CTVS ) - regressed dogs were more cytotoxic against CTVS cells than non-sensitized PBL from untreated dogs .
	manualset3
132994	3	406704	5	NULL	NULL	0	NULL	regressed dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitized peripheral blood lymphocytes ( PBL ) obtained from canine transmissible venereal sarcoma ( CTVS ) - regressed dogs were more cytotoxic against CTVS cells than non-sensitized PBL from untreated dogs .
	manualset3
132996	5	406704	5	NULL	NULL	0	NULL	CTVS cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitized peripheral blood lymphocytes ( PBL ) obtained from canine transmissible venereal sarcoma ( CTVS ) - regressed dogs were more cytotoxic against CTVS cells than non-sensitized PBL from untreated dogs .
	manualset3
132997	6	406704	5	NULL	NULL	0	NULL	non-sensitized PBL	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitized peripheral blood lymphocytes ( PBL ) obtained from canine transmissible venereal sarcoma ( CTVS ) - regressed dogs were more cytotoxic against CTVS cells than non-sensitized PBL from untreated dogs .
	manualset3
132998	7	406704	5	NULL	NULL	0	NULL	untreated dogs 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitized peripheral blood lymphocytes ( PBL ) obtained from canine transmissible venereal sarcoma ( CTVS ) - regressed dogs were more cytotoxic against CTVS cells than non-sensitized PBL from untreated dogs .
	manualset3
132999	1	406705	5	NULL	NULL	NULL	NULL	Sensory assessment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Sensory assessment of epidural block for Caesarean section : a systematic comparison of pinprick , cold and touch sensation .
	manualset3
133000	2	406705	5	NULL	NULL	0	NULL	epidural block	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensory assessment of epidural block for Caesarean section : a systematic comparison of pinprick , cold and touch sensation .
	manualset3
133001	3	406705	5	NULL	NULL	0	NULL	Caesarean section 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensory assessment of epidural block for Caesarean section : a systematic comparison of pinprick , cold and touch sensation .
	manualset3
133002	4	406705	5	NULL	NULL	0	NULL	systematic comparison 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensory assessment of epidural block for Caesarean section : a systematic comparison of pinprick , cold and touch sensation .
	manualset3
133003	5	406705	5	NULL	NULL	0	NULL	pinprick 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensory assessment of epidural block for Caesarean section : a systematic comparison of pinprick , cold and touch sensation .
	manualset3
133004	6	406705	5	NULL	NULL	0	NULL	cold sensation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensory assessment of epidural block for Caesarean section : a systematic comparison of pinprick , cold and touch sensation .
	manualset3
133005	7	406705	5	NULL	NULL	0	NULL	touch sensation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensory assessment of epidural block for Caesarean section : a systematic comparison of pinprick , cold and touch sensation .
	manualset3
133006	1	406706	5	NULL	NULL	0	NULL	Sensory nerve terminations	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensory nerve terminations in the oral tissues of some Pongidae .
	manualset3
133007	2	406706	5	NULL	NULL	0	NULL	oral tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensory nerve terminations in the oral tissues of some Pongidae .
	manualset3
133008	3	406706	5	NULL	NULL	0	NULL	Pongidae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensory nerve terminations in the oral tissues of some Pongidae .
	manualset3
133009	1	406707	5	NULL	NULL	0	NULL	Sensory neuropathy 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensory neuropathy in hereditary spastic paraplegia .
	manualset3
133010	2	406707	5	NULL	NULL	0	NULL	hereditary spastic paraplegia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensory neuropathy in hereditary spastic paraplegia .
	manualset3
133011	1	406708	5	NULL	NULL	0	NULL	Sensory testing 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensory testing of inferior alveolar nerve injuries : a review of methods used in prospective studies .
	manualset3
133012	2	406708	5	NULL	NULL	0	NULL	inferior alveolar nerve injuries	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensory testing of inferior alveolar nerve injuries : a review of methods used in prospective studies .
	manualset3
133013	3	406708	5	NULL	NULL	0	NULL	review 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensory testing of inferior alveolar nerve injuries : a review of methods used in prospective studies .
	manualset3
133014	4	406708	5	NULL	NULL	0	NULL	methods 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensory testing of inferior alveolar nerve injuries : a review of methods used in prospective studies .
	manualset3
133015	5	406708	5	NULL	NULL	0	NULL	prospective studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensory testing of inferior alveolar nerve injuries : a review of methods used in prospective studies .
	manualset3
133016	1	406709	5	NULL	NULL	0	NULL	epignathi 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Separate epignathi of the mandible and the nasopharynx with cleft palate : case report .
	manualset3
133017	2	406709	5	NULL	NULL	0	NULL	mandible 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Separate epignathi of the mandible and the nasopharynx with cleft palate : case report .
	manualset3
133018	3	406709	5	NULL	NULL	0	NULL	nasopharynx 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Separate epignathi of the mandible and the nasopharynx with cleft palate : case report .
	manualset3
133019	4	406709	5	NULL	NULL	0	NULL	cleft palate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Separate epignathi of the mandible and the nasopharynx with cleft palate : case report .
	manualset3
133020	5	406709	5	NULL	NULL	0	NULL	case report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Separate epignathi of the mandible and the nasopharynx with cleft palate : case report .
	manualset3
133021	1	406710	5	NULL	NULL	0	NULL	nephelometric assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new nephelometric assay for beta-trace protein ( prostaglandin D synthase ) as an indicator of liquorrhoea .
	manualset3
133022	2	406710	5	NULL	NULL	0	NULL	beta-trace protein ( prostaglandin D synthase )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A new nephelometric assay for beta-trace protein ( prostaglandin D synthase ) as an indicator of liquorrhoea .
	manualset3
133023	3	406710	5	NULL	NULL	0	NULL	indicator 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new nephelometric assay for beta-trace protein ( prostaglandin D synthase ) as an indicator of liquorrhoea .
	manualset3
133024	4	406710	5	NULL	NULL	0	NULL	liquorrhoea 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A new nephelometric assay for beta-trace protein ( prostaglandin D synthase ) as an indicator of liquorrhoea .
	manualset3
133025	1	406711	5	NULL	NULL	0	NULL	Separation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Separation is enhanced by addition of an electrolyte ( NaCl ) .
	manualset3
133026	2	406711	5	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Separation is enhanced by addition of an electrolyte ( NaCl ) .
	manualset3
133027	3	406711	5	NULL	NULL	0	NULL	electrolyte ( NaCl )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Separation is enhanced by addition of an electrolyte ( NaCl ) .
	manualset3
133028	1	406712	5	NULL	NULL	0	NULL	Separation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Separation of HL-A2 from a mixture of HL-A7 and HL-A12 was achieved on the final DEAE-cellulose column .
	manualset3
133029	2	406712	5	NULL	NULL	0	NULL	HL-A2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Separation of HL-A2 from a mixture of HL-A7 and HL-A12 was achieved on the final DEAE-cellulose column .
	manualset3
133030	3	406712	5	NULL	NULL	0	NULL	mixture	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Separation of HL-A2 from a mixture of HL-A7 and HL-A12 was achieved on the final DEAE-cellulose column .
	manualset3
133031	4	406712	5	NULL	NULL	0	NULL	HL-A7	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Separation of HL-A2 from a mixture of HL-A7 and HL-A12 was achieved on the final DEAE-cellulose column .
	manualset3
133032	5	406712	5	NULL	NULL	0	NULL	HL-A12	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Separation of HL-A2 from a mixture of HL-A7 and HL-A12 was achieved on the final DEAE-cellulose column .
	manualset3
133033	6	406712	5	NULL	NULL	0	NULL	DEAE-cellulose column	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Separation of HL-A2 from a mixture of HL-A7 and HL-A12 was achieved on the final DEAE-cellulose column .
	manualset3
133034	1	406713	5	NULL	NULL	0	NULL	Separation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Separation of the enantiomers of beta-receptor blocking agents and other cationic drugs using a CHIRAL-AGP column .
	manualset3
133035	2	406713	5	NULL	NULL	0	NULL	enantiomers 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Separation of the enantiomers of beta-receptor blocking agents and other cationic drugs using a CHIRAL-AGP column .
	manualset3
133036	3	406713	5	NULL	NULL	0	NULL	beta-receptor blocking agents	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Separation of the enantiomers of beta-receptor blocking agents and other cationic drugs using a CHIRAL-AGP column .
	manualset3
133037	4	406713	5	NULL	NULL	0	NULL	cationic drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Separation of the enantiomers of beta-receptor blocking agents and other cationic drugs using a CHIRAL-AGP column .
	manualset3
133038	5	406713	5	NULL	NULL	0	NULL	CHIRAL-AGP column	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Separation of the enantiomers of beta-receptor blocking agents and other cationic drugs using a CHIRAL-AGP column .
	manualset3
133039	1	406714	5	NULL	NULL	0	NULL	Sephadex	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sephadex alone increased the total number of apoptotic cells , which were not efficiently engulfed by macrophages or other cells , in vivo .
	manualset3
133040	2	406714	5	NULL	NULL	0	NULL	total number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sephadex alone increased the total number of apoptotic cells , which were not efficiently engulfed by macrophages or other cells , in vivo .
	manualset3
133041	3	406714	5	NULL	NULL	0	NULL	apoptotic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Sephadex alone increased the total number of apoptotic cells , which were not efficiently engulfed by macrophages or other cells , in vivo .
	manualset3
133042	4	406714	5	NULL	NULL	0	NULL	macrophages 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Sephadex alone increased the total number of apoptotic cells , which were not efficiently engulfed by macrophages or other cells , in vivo .
	manualset3
133043	5	406714	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Sephadex alone increased the total number of apoptotic cells , which were not efficiently engulfed by macrophages or other cells , in vivo .
	manualset3
133044	1	406715	5	NULL	NULL	0	NULL	Sepharose-AT chromatography 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sepharose-AT chromatography of the ATH component with short heparin chains ( & lt ; or = 12 monosaccharides ) resulted in active unbound ( 40 % ) and bound fractions ( 190 and 560 units/mg , respectively ) .
	manualset3
133045	2	406715	5	NULL	NULL	0	NULL	ATH component	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sepharose-AT chromatography of the ATH component with short heparin chains ( & lt ; or = 12 monosaccharides ) resulted in active unbound ( 40 % ) and bound fractions ( 190 and 560 units/mg , respectively ) .
	manualset3
133046	3	406715	5	NULL	NULL	0	NULL	short heparin chains	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Sepharose-AT chromatography of the ATH component with short heparin chains ( & lt ; or = 12 monosaccharides ) resulted in active unbound ( 40 % ) and bound fractions ( 190 and 560 units/mg , respectively ) .
	manualset3
133047	4	406715	5	NULL	NULL	0	NULL	& lt ; or = 12 monosaccharides	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sepharose-AT chromatography of the ATH component with short heparin chains ( & lt ; or = 12 monosaccharides ) resulted in active unbound ( 40 % ) and bound fractions ( 190 and 560 units/mg , respectively ) .
	manualset3
133048	5	406715	5	NULL	NULL	0	NULL	active unbound fractions	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Sepharose-AT chromatography of the ATH component with short heparin chains ( & lt ; or = 12 monosaccharides ) resulted in active unbound ( 40 % ) and bound fractions ( 190 and 560 units/mg , respectively ) .
	manualset3
133049	6	406715	5	NULL	NULL	0	NULL	 40 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sepharose-AT chromatography of the ATH component with short heparin chains ( & lt ; or = 12 monosaccharides ) resulted in active unbound ( 40 % ) and bound fractions ( 190 and 560 units/mg , respectively ) .
	manualset3
133050	7	406715	5	NULL	NULL	0	NULL	bound fractions	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Sepharose-AT chromatography of the ATH component with short heparin chains ( & lt ; or = 12 monosaccharides ) resulted in active unbound ( 40 % ) and bound fractions ( 190 and 560 units/mg , respectively ) .
	manualset3
133051	8	406715	5	NULL	NULL	0	NULL	190 and 560 units/mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sepharose-AT chromatography of the ATH component with short heparin chains ( & lt ; or = 12 monosaccharides ) resulted in active unbound ( 40 % ) and bound fractions ( 190 and 560 units/mg , respectively ) .
	manualset3
133052	1	406716	5	NULL	NULL	0	NULL	Sepsis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sepsis is a frequent complication of central venous catheters , but the diagnosis of catheter sepsis is not always clear-cut .
	manualset3
133053	2	406716	5	NULL	NULL	0	NULL	frequent complication 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sepsis is a frequent complication of central venous catheters , but the diagnosis of catheter sepsis is not always clear-cut .
	manualset3
133054	3	406716	5	NULL	NULL	0	NULL	central venous catheters 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Sepsis is a frequent complication of central venous catheters , but the diagnosis of catheter sepsis is not always clear-cut .
	manualset3
133055	4	406716	5	NULL	NULL	0	NULL	diagnosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sepsis is a frequent complication of central venous catheters , but the diagnosis of catheter sepsis is not always clear-cut .
	manualset3
133056	5	406716	5	NULL	NULL	0	NULL	catheter sepsis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sepsis is a frequent complication of central venous catheters , but the diagnosis of catheter sepsis is not always clear-cut .
	manualset3
133057	1	406717	5	NULL	NULL	0	NULL	Septic arthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Septic arthritis of the sternoclavicular joint ( SCJ ) is a rare condition speculated to be associated with some predisposing factors such as intravenous drug use , immunocompromised situations or chronic diseases .
	manualset3
133058	2	406717	5	NULL	NULL	0	NULL	sternoclavicular joint ( SCJ ) 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Septic arthritis of the sternoclavicular joint ( SCJ ) is a rare condition speculated to be associated with some predisposing factors such as intravenous drug use , immunocompromised situations or chronic diseases .
	manualset3
133059	3	406717	5	NULL	NULL	0	NULL	rare condition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Septic arthritis of the sternoclavicular joint ( SCJ ) is a rare condition speculated to be associated with some predisposing factors such as intravenous drug use , immunocompromised situations or chronic diseases .
	manualset3
133060	4	406717	5	NULL	NULL	0	NULL	predisposing factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Septic arthritis of the sternoclavicular joint ( SCJ ) is a rare condition speculated to be associated with some predisposing factors such as intravenous drug use , immunocompromised situations or chronic diseases .
	manualset3
133061	5	406717	5	NULL	NULL	NULL	NULL	intravenous drug use	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Septic arthritis of the sternoclavicular joint ( SCJ ) is a rare condition speculated to be associated with some predisposing factors such as intravenous drug use , immunocompromised situations or chronic diseases .
	manualset3
133062	6	406717	5	NULL	NULL	0	NULL	immunocompromised situations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Septic arthritis of the sternoclavicular joint ( SCJ ) is a rare condition speculated to be associated with some predisposing factors such as intravenous drug use , immunocompromised situations or chronic diseases .
	manualset3
133063	7	406717	5	NULL	NULL	0	NULL	chronic diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Septic arthritis of the sternoclavicular joint ( SCJ ) is a rare condition speculated to be associated with some predisposing factors such as intravenous drug use , immunocompromised situations or chronic diseases .
	manualset3
133064	1	406718	5	NULL	NULL	0	NULL	SeqAnt	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	SeqAnt : a web service to rapidly identify and annotate DNA sequence variations .
	manualset3
133065	2	406718	5	NULL	NULL	0	NULL	web service	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	SeqAnt : a web service to rapidly identify and annotate DNA sequence variations .
	manualset3
133066	3	406718	5	NULL	NULL	0	NULL	DNA sequence variations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SeqAnt : a web service to rapidly identify and annotate DNA sequence variations .
	manualset3
133067	1	406719	5	NULL	NULL	0	NULL	new rapid high-performance liquid chromatographic method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A new rapid high-performance liquid chromatographic method , without urine sample pre-treatment and based on isocratic ion-pair elution , fluorimetric detection and column-switching , has been developed for the determination of vanillylmandelic acid .
	manualset3
133068	2	406719	5	NULL	NULL	0	NULL	urine sample pre-treatment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new rapid high-performance liquid chromatographic method , without urine sample pre-treatment and based on isocratic ion-pair elution , fluorimetric detection and column-switching , has been developed for the determination of vanillylmandelic acid .
	manualset3
133069	3	406719	5	NULL	NULL	0	NULL	isocratic ion-pair elution	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new rapid high-performance liquid chromatographic method , without urine sample pre-treatment and based on isocratic ion-pair elution , fluorimetric detection and column-switching , has been developed for the determination of vanillylmandelic acid .
	manualset3
133070	4	406719	5	NULL	NULL	0	NULL	fluorimetric detection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new rapid high-performance liquid chromatographic method , without urine sample pre-treatment and based on isocratic ion-pair elution , fluorimetric detection and column-switching , has been developed for the determination of vanillylmandelic acid .
	manualset3
133071	5	406719	5	NULL	NULL	0	NULL	column-switching	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new rapid high-performance liquid chromatographic method , without urine sample pre-treatment and based on isocratic ion-pair elution , fluorimetric detection and column-switching , has been developed for the determination of vanillylmandelic acid .
	manualset3
133072	6	406719	5	NULL	NULL	0	NULL	determination 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new rapid high-performance liquid chromatographic method , without urine sample pre-treatment and based on isocratic ion-pair elution , fluorimetric detection and column-switching , has been developed for the determination of vanillylmandelic acid .
	manualset3
133073	7	406719	5	NULL	NULL	0	NULL	vanillylmandelic acid	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A new rapid high-performance liquid chromatographic method , without urine sample pre-treatment and based on isocratic ion-pair elution , fluorimetric detection and column-switching , has been developed for the determination of vanillylmandelic acid .
	manualset3
133074	1	406720	5	NULL	NULL	0	NULL	Sequence alignment analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence alignment analysis was further conducted with different groups of flaviviruses to show that the prM H99 residues are generally conserved .
	manualset3
133075	2	406720	5	NULL	NULL	0	NULL	groups 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence alignment analysis was further conducted with different groups of flaviviruses to show that the prM H99 residues are generally conserved .
	manualset3
133076	3	406720	5	NULL	NULL	0	NULL	flaviviruses 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence alignment analysis was further conducted with different groups of flaviviruses to show that the prM H99 residues are generally conserved .
	manualset3
133077	4	406720	5	NULL	NULL	0	NULL	prM H99 residues 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence alignment analysis was further conducted with different groups of flaviviruses to show that the prM H99 residues are generally conserved .
	manualset3
133078	1	406721	5	NULL	NULL	0	NULL	Sequence analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence analysis and PCR-RFLP profiling of the hsp70 gene as a valuable tool for identifying Leishmania species associated with human leishmaniasis in Brazil .
	manualset3
133079	2	406721	5	NULL	NULL	0	NULL	 PCR-RFLP profiling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence analysis and PCR-RFLP profiling of the hsp70 gene as a valuable tool for identifying Leishmania species associated with human leishmaniasis in Brazil .
	manualset3
133080	3	406721	5	NULL	NULL	0	NULL	hsp70 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence analysis and PCR-RFLP profiling of the hsp70 gene as a valuable tool for identifying Leishmania species associated with human leishmaniasis in Brazil .
	manualset3
133081	4	406721	5	NULL	NULL	0	NULL	valuable tool	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence analysis and PCR-RFLP profiling of the hsp70 gene as a valuable tool for identifying Leishmania species associated with human leishmaniasis in Brazil .
	manualset3
133082	5	406721	5	NULL	NULL	0	NULL	Leishmania species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence analysis and PCR-RFLP profiling of the hsp70 gene as a valuable tool for identifying Leishmania species associated with human leishmaniasis in Brazil .
	manualset3
133083	6	406721	5	NULL	NULL	0	NULL	human leishmaniasis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence analysis and PCR-RFLP profiling of the hsp70 gene as a valuable tool for identifying Leishmania species associated with human leishmaniasis in Brazil .
	manualset3
133084	7	406721	5	NULL	NULL	0	NULL	Brazil 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence analysis and PCR-RFLP profiling of the hsp70 gene as a valuable tool for identifying Leishmania species associated with human leishmaniasis in Brazil .
	manualset3
133085	1	406722	5	NULL	NULL	0	NULL	Sequence analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence analysis of cloned PCR-amplified narG , napA , and nrfA gene sequences showed the indigenous nitrate-reducing communities to be both phylogenetically diverse and also divergent from previously characterized nitrate reduction sequences in soils and offshore marine sediments and from cultured nitrate reducers .
	manualset3
133086	2	406722	5	NULL	NULL	0	NULL	cloned PCR-amplified narG gene sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence analysis of cloned PCR-amplified narG , napA , and nrfA gene sequences showed the indigenous nitrate-reducing communities to be both phylogenetically diverse and also divergent from previously characterized nitrate reduction sequences in soils and offshore marine sediments and from cultured nitrate reducers .
	manualset3
133087	3	406722	5	NULL	NULL	0	NULL	cloned PCR-amplified napA gene sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence analysis of cloned PCR-amplified narG , napA , and nrfA gene sequences showed the indigenous nitrate-reducing communities to be both phylogenetically diverse and also divergent from previously characterized nitrate reduction sequences in soils and offshore marine sediments and from cultured nitrate reducers .
	manualset3
133088	4	406722	5	NULL	NULL	0	NULL	cloned PCR-amplified  nrfA gene sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence analysis of cloned PCR-amplified narG , napA , and nrfA gene sequences showed the indigenous nitrate-reducing communities to be both phylogenetically diverse and also divergent from previously characterized nitrate reduction sequences in soils and offshore marine sediments and from cultured nitrate reducers .
	manualset3
133089	5	406722	5	NULL	NULL	0	NULL	indigenous nitrate-reducing communities	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence analysis of cloned PCR-amplified narG , napA , and nrfA gene sequences showed the indigenous nitrate-reducing communities to be both phylogenetically diverse and also divergent from previously characterized nitrate reduction sequences in soils and offshore marine sediments and from cultured nitrate reducers .
	manualset3
133090	6	406722	5	NULL	NULL	0	NULL	nitrate reduction sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence analysis of cloned PCR-amplified narG , napA , and nrfA gene sequences showed the indigenous nitrate-reducing communities to be both phylogenetically diverse and also divergent from previously characterized nitrate reduction sequences in soils and offshore marine sediments and from cultured nitrate reducers .
	manualset3
133091	7	406722	5	NULL	NULL	0	NULL	soils 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence analysis of cloned PCR-amplified narG , napA , and nrfA gene sequences showed the indigenous nitrate-reducing communities to be both phylogenetically diverse and also divergent from previously characterized nitrate reduction sequences in soils and offshore marine sediments and from cultured nitrate reducers .
	manualset3
133092	8	406722	5	NULL	NULL	0	NULL	offshore marine sediments	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence analysis of cloned PCR-amplified narG , napA , and nrfA gene sequences showed the indigenous nitrate-reducing communities to be both phylogenetically diverse and also divergent from previously characterized nitrate reduction sequences in soils and offshore marine sediments and from cultured nitrate reducers .
	manualset3
133093	9	406722	5	NULL	NULL	0	NULL	cultured nitrate reducers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence analysis of cloned PCR-amplified narG , napA , and nrfA gene sequences showed the indigenous nitrate-reducing communities to be both phylogenetically diverse and also divergent from previously characterized nitrate reduction sequences in soils and offshore marine sediments and from cultured nitrate reducers .
	manualset3
133094	1	406723	5	NULL	NULL	0	NULL	Sequence analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence analysis of the amplified product revealed a GAG ) AAG transversion at codon 26 , which resulted in an amino acid substitution of lysine for glutamic acid .
	manualset3
133095	2	406723	5	NULL	NULL	0	NULL	amplified product 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence analysis of the amplified product revealed a GAG ) AAG transversion at codon 26 , which resulted in an amino acid substitution of lysine for glutamic acid .
	manualset3
133096	3	406723	5	NULL	NULL	0	NULL	 GAG ) AAG transversion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence analysis of the amplified product revealed a GAG ) AAG transversion at codon 26 , which resulted in an amino acid substitution of lysine for glutamic acid .
	manualset3
133097	4	406723	5	NULL	NULL	0	NULL	codon 26	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence analysis of the amplified product revealed a GAG ) AAG transversion at codon 26 , which resulted in an amino acid substitution of lysine for glutamic acid .
	manualset3
133098	5	406723	5	NULL	NULL	0	NULL	amino acid substitution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence analysis of the amplified product revealed a GAG ) AAG transversion at codon 26 , which resulted in an amino acid substitution of lysine for glutamic acid .
	manualset3
133099	6	406723	5	NULL	NULL	0	NULL	lysine 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence analysis of the amplified product revealed a GAG ) AAG transversion at codon 26 , which resulted in an amino acid substitution of lysine for glutamic acid .
	manualset3
133100	7	406723	5	NULL	NULL	NULL	NULL	glutamic acid	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Sequence analysis of the amplified product revealed a GAG ) AAG transversion at codon 26 , which resulted in an amino acid substitution of lysine for glutamic acid .
	manualset3
133101	1	406724	5	NULL	NULL	0	NULL	Sequence analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence analysis of the proximal 5 ' - flanking region of the gene reveals the existence of a TATA box appropriately located with respect to the transcription initiation site and several potential cis-regulatory elements that might contribute to the transcriptional regulation of the CD36 gene .
	manualset3
133102	2	406724	5	NULL	NULL	0	NULL	proximal 5 ' - flanking region 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence analysis of the proximal 5 ' - flanking region of the gene reveals the existence of a TATA box appropriately located with respect to the transcription initiation site and several potential cis-regulatory elements that might contribute to the transcriptional regulation of the CD36 gene .
	manualset3
133103	3	406724	5	NULL	NULL	0	NULL	gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence analysis of the proximal 5 ' - flanking region of the gene reveals the existence of a TATA box appropriately located with respect to the transcription initiation site and several potential cis-regulatory elements that might contribute to the transcriptional regulation of the CD36 gene .
	manualset3
133104	4	406724	5	NULL	NULL	0	NULL	TATA box	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence analysis of the proximal 5 ' - flanking region of the gene reveals the existence of a TATA box appropriately located with respect to the transcription initiation site and several potential cis-regulatory elements that might contribute to the transcriptional regulation of the CD36 gene .
	manualset3
133105	5	406724	5	NULL	NULL	0	NULL	transcription initiation site 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence analysis of the proximal 5 ' - flanking region of the gene reveals the existence of a TATA box appropriately located with respect to the transcription initiation site and several potential cis-regulatory elements that might contribute to the transcriptional regulation of the CD36 gene .
	manualset3
133106	6	406724	5	NULL	NULL	0	NULL	potential cis-regulatory elements	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence analysis of the proximal 5 ' - flanking region of the gene reveals the existence of a TATA box appropriately located with respect to the transcription initiation site and several potential cis-regulatory elements that might contribute to the transcriptional regulation of the CD36 gene .
	manualset3
133107	7	406724	5	NULL	NULL	0	NULL	transcriptional regulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence analysis of the proximal 5 ' - flanking region of the gene reveals the existence of a TATA box appropriately located with respect to the transcription initiation site and several potential cis-regulatory elements that might contribute to the transcriptional regulation of the CD36 gene .
	manualset3
133108	8	406724	5	NULL	NULL	0	NULL	 CD36 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence analysis of the proximal 5 ' - flanking region of the gene reveals the existence of a TATA box appropriately located with respect to the transcription initiation site and several potential cis-regulatory elements that might contribute to the transcriptional regulation of the CD36 gene .
	manualset3
133109	1	406725	5	NULL	NULL	0	NULL	Sequence and structural analyses 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence and structural analyses reveal that DOHH belongs to a family of HEAT-repeat-containing proteins , consisting of eight tandem repeats of an alpha-helical pair ( HEAT motif ) organized in a symmetrical dyad .
	manualset3
133110	2	406725	5	NULL	NULL	0	NULL	DOHH 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence and structural analyses reveal that DOHH belongs to a family of HEAT-repeat-containing proteins , consisting of eight tandem repeats of an alpha-helical pair ( HEAT motif ) organized in a symmetrical dyad .
	manualset3
133111	3	406725	5	NULL	NULL	0	NULL	family of HEAT-repeat-containing proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence and structural analyses reveal that DOHH belongs to a family of HEAT-repeat-containing proteins , consisting of eight tandem repeats of an alpha-helical pair ( HEAT motif ) organized in a symmetrical dyad .
	manualset3
133112	4	406725	5	NULL	NULL	0	NULL	eight 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence and structural analyses reveal that DOHH belongs to a family of HEAT-repeat-containing proteins , consisting of eight tandem repeats of an alpha-helical pair ( HEAT motif ) organized in a symmetrical dyad .
	manualset3
133113	5	406725	5	NULL	NULL	NULL	NULL	tandem repeats of an alpha-helical pair ( HEAT motif ) 	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Sequence and structural analyses reveal that DOHH belongs to a family of HEAT-repeat-containing proteins , consisting of eight tandem repeats of an alpha-helical pair ( HEAT motif ) organized in a symmetrical dyad .
	manualset3
133114	6	406725	5	NULL	NULL	0	NULL	symmetrical dyad 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence and structural analyses reveal that DOHH belongs to a family of HEAT-repeat-containing proteins , consisting of eight tandem repeats of an alpha-helical pair ( HEAT motif ) organized in a symmetrical dyad .
	manualset3
133115	1	406726	5	NULL	NULL	0	NULL	Sequence characterization 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence characterization , polymorphism , and chromosomal localizations of the porcine CapZ genes .
	manualset3
133116	2	406726	5	NULL	NULL	0	NULL	polymorphism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence characterization , polymorphism , and chromosomal localizations of the porcine CapZ genes .
	manualset3
133117	3	406726	5	NULL	NULL	0	NULL	chromosomal localizations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence characterization , polymorphism , and chromosomal localizations of the porcine CapZ genes .
	manualset3
133118	4	406726	5	NULL	NULL	0	NULL	porcine CapZ genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence characterization , polymorphism , and chromosomal localizations of the porcine CapZ genes .
	manualset3
133119	1	406727	5	NULL	NULL	0	NULL	Sequence organization 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence organization and transcription at two heat shock loci in Drosophila .
	manualset3
133120	2	406727	5	NULL	NULL	0	NULL	transcription 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence organization and transcription at two heat shock loci in Drosophila .
	manualset3
133121	3	406727	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence organization and transcription at two heat shock loci in Drosophila .
	manualset3
133122	4	406727	5	NULL	NULL	0	NULL	heat shock loci	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence organization and transcription at two heat shock loci in Drosophila .
	manualset3
133123	5	406727	5	NULL	NULL	0	NULL	Drosophila 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence organization and transcription at two heat shock loci in Drosophila .
	manualset3
133124	1	406728	5	NULL	NULL	0	NULL	Sequence rearrangements	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence rearrangements and genome instability .
	manualset3
133125	2	406728	5	NULL	NULL	0	NULL	genome instability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence rearrangements and genome instability .
	manualset3
133126	1	406729	5	NULL	NULL	0	NULL	Sequence similarity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence similarity to cDNA53 is located in at least five chromosomes , and its small chromosome copy is a pseudogene .
	manualset3
133127	2	406729	5	NULL	NULL	0	NULL	cDNA53 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence similarity to cDNA53 is located in at least five chromosomes , and its small chromosome copy is a pseudogene .
	manualset3
133128	3	406729	5	NULL	NULL	0	NULL	five 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence similarity to cDNA53 is located in at least five chromosomes , and its small chromosome copy is a pseudogene .
	manualset3
133129	4	406729	5	NULL	NULL	0	NULL	chromosomes 	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence similarity to cDNA53 is located in at least five chromosomes , and its small chromosome copy is a pseudogene .
	manualset3
133130	5	406729	5	NULL	NULL	0	NULL	small chromosome copy 	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence similarity to cDNA53 is located in at least five chromosomes , and its small chromosome copy is a pseudogene .
	manualset3
133131	6	406729	5	NULL	NULL	0	NULL	pseudogene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence similarity to cDNA53 is located in at least five chromosomes , and its small chromosome copy is a pseudogene .
	manualset3
133158	1	406730	5	NULL	NULL	0	NULL	Sequences 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequences have been annotated via BLAST match results and using Gene Ontology terms .
	manualset3
133159	2	406730	5	NULL	NULL	0	NULL	BLAST match results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequences have been annotated via BLAST match results and using Gene Ontology terms .
	manualset3
133160	3	406730	5	NULL	NULL	0	NULL	Gene Ontology terms	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequences have been annotated via BLAST match results and using Gene Ontology terms .
	manualset3
133161	1	406731	5	NULL	NULL	0	NULL	Sequencing 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequencing , mass spectrometry , and analytical isoelectrofocusing indicated the existence of isoforms , as reported for other PLIalphas isolated from snake plasma .
	manualset3
133162	2	406731	5	NULL	NULL	0	NULL	mass spectrometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequencing , mass spectrometry , and analytical isoelectrofocusing indicated the existence of isoforms , as reported for other PLIalphas isolated from snake plasma .
	manualset3
133163	3	406731	5	NULL	NULL	0	NULL	analytical isoelectrofocusing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequencing , mass spectrometry , and analytical isoelectrofocusing indicated the existence of isoforms , as reported for other PLIalphas isolated from snake plasma .
	manualset3
133164	4	406731	5	NULL	NULL	0	NULL	isoforms 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequencing , mass spectrometry , and analytical isoelectrofocusing indicated the existence of isoforms , as reported for other PLIalphas isolated from snake plasma .
	manualset3
133167	5	406731	5	NULL	NULL	0	NULL	PLIalphas	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequencing , mass spectrometry , and analytical isoelectrofocusing indicated the existence of isoforms , as reported for other PLIalphas isolated from snake plasma .
	manualset3
133170	6	406731	5	NULL	NULL	0	NULL	snake plasma	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequencing , mass spectrometry , and analytical isoelectrofocusing indicated the existence of isoforms , as reported for other PLIalphas isolated from snake plasma .
	manualset3
133177	1	406732	5	NULL	NULL	0	NULL	 2 , 951 nucleotides	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequencing 2 , 951 nucleotides of the 3 ' proximal region of the genome of a potyvirus isolate collected from Capsicum pubescens ( rocoto ) pepper in Ecuador revealed that this was the first representative of a new species tentatively named Ecuadorian rocoto virus ( ERV ) .
	manualset3
133178	2	406732	5	NULL	NULL	0	NULL	3 ' proximal region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequencing 2 , 951 nucleotides of the 3 ' proximal region of the genome of a potyvirus isolate collected from Capsicum pubescens ( rocoto ) pepper in Ecuador revealed that this was the first representative of a new species tentatively named Ecuadorian rocoto virus ( ERV ) .
	manualset3
133179	3	406732	5	NULL	NULL	0	NULL	genome 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequencing 2 , 951 nucleotides of the 3 ' proximal region of the genome of a potyvirus isolate collected from Capsicum pubescens ( rocoto ) pepper in Ecuador revealed that this was the first representative of a new species tentatively named Ecuadorian rocoto virus ( ERV ) .
	manualset3
133181	4	406732	5	NULL	NULL	0	NULL	potyvirus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequencing 2 , 951 nucleotides of the 3 ' proximal region of the genome of a potyvirus isolate collected from Capsicum pubescens ( rocoto ) pepper in Ecuador revealed that this was the first representative of a new species tentatively named Ecuadorian rocoto virus ( ERV ) .
	manualset3
133182	5	406732	5	NULL	NULL	0	NULL	Capsicum pubescens ( rocoto ) pepper	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequencing 2 , 951 nucleotides of the 3 ' proximal region of the genome of a potyvirus isolate collected from Capsicum pubescens ( rocoto ) pepper in Ecuador revealed that this was the first representative of a new species tentatively named Ecuadorian rocoto virus ( ERV ) .
	manualset3
133183	6	406732	5	NULL	NULL	0	NULL	Ecuador 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequencing 2 , 951 nucleotides of the 3 ' proximal region of the genome of a potyvirus isolate collected from Capsicum pubescens ( rocoto ) pepper in Ecuador revealed that this was the first representative of a new species tentatively named Ecuadorian rocoto virus ( ERV ) .
	manualset3
133184	7	406732	5	NULL	NULL	0	NULL	first representative	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequencing 2 , 951 nucleotides of the 3 ' proximal region of the genome of a potyvirus isolate collected from Capsicum pubescens ( rocoto ) pepper in Ecuador revealed that this was the first representative of a new species tentatively named Ecuadorian rocoto virus ( ERV ) .
	manualset3
133185	8	406732	5	NULL	NULL	0	NULL	new species 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequencing 2 , 951 nucleotides of the 3 ' proximal region of the genome of a potyvirus isolate collected from Capsicum pubescens ( rocoto ) pepper in Ecuador revealed that this was the first representative of a new species tentatively named Ecuadorian rocoto virus ( ERV ) .
	manualset3
133186	9	406732	5	NULL	NULL	0	NULL	Ecuadorian rocoto virus ( ERV )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequencing 2 , 951 nucleotides of the 3 ' proximal region of the genome of a potyvirus isolate collected from Capsicum pubescens ( rocoto ) pepper in Ecuador revealed that this was the first representative of a new species tentatively named Ecuadorian rocoto virus ( ERV ) .
	manualset3
133189	1	406733	5	NULL	NULL	0	NULL	5-fluorouracil	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential 5-fluorouracil and leucovorin in patients with advanced symptomatic gastrointestinal cancer .
	manualset3
133190	2	406733	5	NULL	NULL	0	NULL	leucovorin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential 5-fluorouracil and leucovorin in patients with advanced symptomatic gastrointestinal cancer .
	manualset3
133191	3	406733	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential 5-fluorouracil and leucovorin in patients with advanced symptomatic gastrointestinal cancer .
	manualset3
133192	4	406733	5	NULL	NULL	0	NULL	advanced symptomatic gastrointestinal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential 5-fluorouracil and leucovorin in patients with advanced symptomatic gastrointestinal cancer .
	manualset3
133194	1	406734	5	NULL	NULL	0	NULL	Sequential Organ Failure Assessment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential Organ Failure Assessment was used to evaluate severity of illness .
	manualset3
133195	2	406734	5	NULL	NULL	0	NULL	severity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential Organ Failure Assessment was used to evaluate severity of illness .
	manualset3
133196	3	406734	5	NULL	NULL	0	NULL	illness 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential Organ Failure Assessment was used to evaluate severity of illness .
	manualset3
133197	1	406735	5	NULL	NULL	0	NULL	Sequential acquisition 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential acquisition of mitochondrial and plasma membrane alterations during early lymphocyte apoptosis .
	manualset3
133199	2	406735	5	NULL	NULL	0	NULL	mitochondrial membrane alterations 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential acquisition of mitochondrial and plasma membrane alterations during early lymphocyte apoptosis .
	manualset3
133201	3	406735	5	NULL	NULL	0	NULL	plasma membrane alterations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential acquisition of mitochondrial and plasma membrane alterations during early lymphocyte apoptosis .
	manualset3
133203	4	406735	5	NULL	NULL	0	NULL	early lymphocyte apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential acquisition of mitochondrial and plasma membrane alterations during early lymphocyte apoptosis .
	manualset3
133204	1	406736	5	NULL	NULL	0	NULL	Case 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( Case of neuromyelitis optica suspected to be toxoplasmosis ) .
	manualset3
133205	2	406736	5	NULL	NULL	0	NULL	neuromyelitis optica 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Case of neuromyelitis optica suspected to be toxoplasmosis ) .
	manualset3
133206	3	406736	5	NULL	NULL	0	NULL	toxoplasmosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Case of neuromyelitis optica suspected to be toxoplasmosis ) .
	manualset3
133207	1	406737	5	NULL	NULL	0	NULL	 solid-contact ion-selective electrode	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A new solid-contact ion-selective electrode has been developed for determining choline and derivatives in aqueous solutions .
	manualset3
133210	2	406737	5	NULL	NULL	0	NULL	choline 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A new solid-contact ion-selective electrode has been developed for determining choline and derivatives in aqueous solutions .
	manualset3
133212	3	406737	5	NULL	NULL	0	NULL	derivatives 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A new solid-contact ion-selective electrode has been developed for determining choline and derivatives in aqueous solutions .
	manualset3
133214	4	406737	5	NULL	NULL	0	NULL	aqueous solutions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A new solid-contact ion-selective electrode has been developed for determining choline and derivatives in aqueous solutions .
	manualset3
133219	1	406738	5	NULL	NULL	0	NULL	Sequential alterations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential alterations of microRNA expression in hepatocellular carcinoma development and venous metastasis .
	manualset3
133220	2	406738	5	NULL	NULL	0	NULL	microRNA expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential alterations of microRNA expression in hepatocellular carcinoma development and venous metastasis .
	manualset3
133221	3	406738	5	NULL	NULL	0	NULL	hepatocellular carcinoma development	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential alterations of microRNA expression in hepatocellular carcinoma development and venous metastasis .
	manualset3
133223	4	406738	5	NULL	NULL	0	NULL	venous metastasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential alterations of microRNA expression in hepatocellular carcinoma development and venous metastasis .
	manualset3
133225	1	406739	5	NULL	NULL	0	NULL	Sequential changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential changes in the signal transduction responses of skeletal muscle following food deprivation .
	manualset3
133227	2	406739	5	NULL	NULL	0	NULL	signal transduction responses	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential changes in the signal transduction responses of skeletal muscle following food deprivation .
	manualset3
133228	3	406739	5	NULL	NULL	0	NULL	skeletal muscle	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential changes in the signal transduction responses of skeletal muscle following food deprivation .
	manualset3
133229	4	406739	5	NULL	NULL	0	NULL	food deprivation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential changes in the signal transduction responses of skeletal muscle following food deprivation .
	manualset3
133230	1	406740	5	NULL	NULL	0	NULL	Sequential field potential analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential field potential analysis along the CA3-CA1-subiculum axis revealed that the amplitude of CA3-driven interictal discharges recorded in the presence of 4AP only diminished within the subiculum .
	manualset3
133233	2	406740	5	NULL	NULL	0	NULL	CA3-CA1-subiculum axis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential field potential analysis along the CA3-CA1-subiculum axis revealed that the amplitude of CA3-driven interictal discharges recorded in the presence of 4AP only diminished within the subiculum .
	manualset3
133235	3	406740	5	NULL	NULL	0	NULL	amplitude 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential field potential analysis along the CA3-CA1-subiculum axis revealed that the amplitude of CA3-driven interictal discharges recorded in the presence of 4AP only diminished within the subiculum .
	manualset3
133236	4	406740	5	NULL	NULL	0	NULL	CA3-driven interictal discharges	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential field potential analysis along the CA3-CA1-subiculum axis revealed that the amplitude of CA3-driven interictal discharges recorded in the presence of 4AP only diminished within the subiculum .
	manualset3
133237	5	406740	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential field potential analysis along the CA3-CA1-subiculum axis revealed that the amplitude of CA3-driven interictal discharges recorded in the presence of 4AP only diminished within the subiculum .
	manualset3
133238	6	406740	5	NULL	NULL	0	NULL	4AP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential field potential analysis along the CA3-CA1-subiculum axis revealed that the amplitude of CA3-driven interictal discharges recorded in the presence of 4AP only diminished within the subiculum .
	manualset3
133239	7	406740	5	NULL	NULL	0	NULL	subiculum 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential field potential analysis along the CA3-CA1-subiculum axis revealed that the amplitude of CA3-driven interictal discharges recorded in the presence of 4AP only diminished within the subiculum .
	manualset3
133240	1	406741	5	NULL	NULL	0	NULL	short tandem repeat polymorphisms 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential short tandem repeat polymorphisms on peripheral blood and bone marrow cells documented the persistence of donor engraftment .
	manualset3
133241	2	406741	5	NULL	NULL	0	NULL	peripheral blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential short tandem repeat polymorphisms on peripheral blood and bone marrow cells documented the persistence of donor engraftment .
	manualset3
133242	3	406741	5	NULL	NULL	0	NULL	bone marrow cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential short tandem repeat polymorphisms on peripheral blood and bone marrow cells documented the persistence of donor engraftment .
	manualset3
133243	4	406741	5	NULL	NULL	0	NULL	persistence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential short tandem repeat polymorphisms on peripheral blood and bone marrow cells documented the persistence of donor engraftment .
	manualset3
133244	5	406741	5	NULL	NULL	0	NULL	donor engraftment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential short tandem repeat polymorphisms on peripheral blood and bone marrow cells documented the persistence of donor engraftment .
	manualset3
133250	1	406742	5	NULL	NULL	0	NULL	Sequential sigmatropic rearrangements ( Claisen/Claisen and Claisen/Overman )	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential sigmatropic rearrangements ( Claisen/Claisen and Claisen/Overman ) of enantiopure allylic diols are described .
	manualset3
133251	2	406742	5	NULL	NULL	0	NULL	enantiopure allylic diols	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequential sigmatropic rearrangements ( Claisen/Claisen and Claisen/Overman ) of enantiopure allylic diols are described .
	manualset3
133253	1	406743	5	NULL	NULL	0	NULL	Sequestration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequestration of bacterial lipopolysaccharide by bis ( Args ) gemini compounds .
	manualset3
133254	2	406743	5	NULL	NULL	0	NULL	bacterial lipopolysaccharide	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequestration of bacterial lipopolysaccharide by bis ( Args ) gemini compounds .
	manualset3
133255	3	406743	5	NULL	NULL	0	NULL	bis ( Args ) gemini compounds 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequestration of bacterial lipopolysaccharide by bis ( Args ) gemini compounds .
	manualset3
133259	1	406744	5	NULL	NULL	0	NULL	Sera 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera from patients with primary fibromyalgia ( 223 sera , 210 women ; 13 men ) were analyzed , by immunofluorescence microscopy , for the presence of antibodies directed against cell nuclei ( ANA ) , smooth muscle , mitochondria and other tissue antigens present in cryostat sections of rat organs ( liver , kidney and stomach ) .
	manualset3
133260	2	406744	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera from patients with primary fibromyalgia ( 223 sera , 210 women ; 13 men ) were analyzed , by immunofluorescence microscopy , for the presence of antibodies directed against cell nuclei ( ANA ) , smooth muscle , mitochondria and other tissue antigens present in cryostat sections of rat organs ( liver , kidney and stomach ) .
	manualset3
133261	3	406744	5	NULL	NULL	0	NULL	primary fibromyalgia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera from patients with primary fibromyalgia ( 223 sera , 210 women ; 13 men ) were analyzed , by immunofluorescence microscopy , for the presence of antibodies directed against cell nuclei ( ANA ) , smooth muscle , mitochondria and other tissue antigens present in cryostat sections of rat organs ( liver , kidney and stomach ) .
	manualset3
133262	4	406744	5	NULL	NULL	0	NULL	223 sera	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera from patients with primary fibromyalgia ( 223 sera , 210 women ; 13 men ) were analyzed , by immunofluorescence microscopy , for the presence of antibodies directed against cell nuclei ( ANA ) , smooth muscle , mitochondria and other tissue antigens present in cryostat sections of rat organs ( liver , kidney and stomach ) .
	manualset3
133263	5	406744	5	NULL	NULL	NULL	NULL	210 women	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Sera from patients with primary fibromyalgia ( 223 sera , 210 women ; 13 men ) were analyzed , by immunofluorescence microscopy , for the presence of antibodies directed against cell nuclei ( ANA ) , smooth muscle , mitochondria and other tissue antigens present in cryostat sections of rat organs ( liver , kidney and stomach ) .
	manualset3
133264	6	406744	5	NULL	NULL	0	NULL	13 men	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera from patients with primary fibromyalgia ( 223 sera , 210 women ; 13 men ) were analyzed , by immunofluorescence microscopy , for the presence of antibodies directed against cell nuclei ( ANA ) , smooth muscle , mitochondria and other tissue antigens present in cryostat sections of rat organs ( liver , kidney and stomach ) .
	manualset3
133265	7	406744	5	NULL	NULL	0	NULL	immunofluorescence microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera from patients with primary fibromyalgia ( 223 sera , 210 women ; 13 men ) were analyzed , by immunofluorescence microscopy , for the presence of antibodies directed against cell nuclei ( ANA ) , smooth muscle , mitochondria and other tissue antigens present in cryostat sections of rat organs ( liver , kidney and stomach ) .
	manualset3
133266	8	406744	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera from patients with primary fibromyalgia ( 223 sera , 210 women ; 13 men ) were analyzed , by immunofluorescence microscopy , for the presence of antibodies directed against cell nuclei ( ANA ) , smooth muscle , mitochondria and other tissue antigens present in cryostat sections of rat organs ( liver , kidney and stomach ) .
	manualset3
133267	9	406744	5	NULL	NULL	NULL	NULL	antibodies 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Sera from patients with primary fibromyalgia ( 223 sera , 210 women ; 13 men ) were analyzed , by immunofluorescence microscopy , for the presence of antibodies directed against cell nuclei ( ANA ) , smooth muscle , mitochondria and other tissue antigens present in cryostat sections of rat organs ( liver , kidney and stomach ) .
	manualset3
133268	10	406744	5	NULL	NULL	0	NULL	cell nuclei ( ANA )	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera from patients with primary fibromyalgia ( 223 sera , 210 women ; 13 men ) were analyzed , by immunofluorescence microscopy , for the presence of antibodies directed against cell nuclei ( ANA ) , smooth muscle , mitochondria and other tissue antigens present in cryostat sections of rat organs ( liver , kidney and stomach ) .
	manualset3
133269	11	406744	5	NULL	NULL	0	NULL	smooth muscle	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera from patients with primary fibromyalgia ( 223 sera , 210 women ; 13 men ) were analyzed , by immunofluorescence microscopy , for the presence of antibodies directed against cell nuclei ( ANA ) , smooth muscle , mitochondria and other tissue antigens present in cryostat sections of rat organs ( liver , kidney and stomach ) .
	manualset3
133270	12	406744	5	NULL	NULL	0	NULL	mitochondria	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera from patients with primary fibromyalgia ( 223 sera , 210 women ; 13 men ) were analyzed , by immunofluorescence microscopy , for the presence of antibodies directed against cell nuclei ( ANA ) , smooth muscle , mitochondria and other tissue antigens present in cryostat sections of rat organs ( liver , kidney and stomach ) .
	manualset3
133273	13	406744	5	NULL	NULL	0	NULL	tissue antigens	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera from patients with primary fibromyalgia ( 223 sera , 210 women ; 13 men ) were analyzed , by immunofluorescence microscopy , for the presence of antibodies directed against cell nuclei ( ANA ) , smooth muscle , mitochondria and other tissue antigens present in cryostat sections of rat organs ( liver , kidney and stomach ) .
	manualset3
133275	14	406744	5	NULL	NULL	NULL	NULL	cryostat sections	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Sera from patients with primary fibromyalgia ( 223 sera , 210 women ; 13 men ) were analyzed , by immunofluorescence microscopy , for the presence of antibodies directed against cell nuclei ( ANA ) , smooth muscle , mitochondria and other tissue antigens present in cryostat sections of rat organs ( liver , kidney and stomach ) .
	manualset3
133277	15	406744	5	NULL	NULL	0	NULL	rat organs 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera from patients with primary fibromyalgia ( 223 sera , 210 women ; 13 men ) were analyzed , by immunofluorescence microscopy , for the presence of antibodies directed against cell nuclei ( ANA ) , smooth muscle , mitochondria and other tissue antigens present in cryostat sections of rat organs ( liver , kidney and stomach ) .
	manualset3
133278	16	406744	5	NULL	NULL	0	NULL	liver 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera from patients with primary fibromyalgia ( 223 sera , 210 women ; 13 men ) were analyzed , by immunofluorescence microscopy , for the presence of antibodies directed against cell nuclei ( ANA ) , smooth muscle , mitochondria and other tissue antigens present in cryostat sections of rat organs ( liver , kidney and stomach ) .
	manualset3
133280	17	406744	5	NULL	NULL	0	NULL	kidney 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera from patients with primary fibromyalgia ( 223 sera , 210 women ; 13 men ) were analyzed , by immunofluorescence microscopy , for the presence of antibodies directed against cell nuclei ( ANA ) , smooth muscle , mitochondria and other tissue antigens present in cryostat sections of rat organs ( liver , kidney and stomach ) .
	manualset3
133281	18	406744	5	NULL	NULL	0	NULL	stomach 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera from patients with primary fibromyalgia ( 223 sera , 210 women ; 13 men ) were analyzed , by immunofluorescence microscopy , for the presence of antibodies directed against cell nuclei ( ANA ) , smooth muscle , mitochondria and other tissue antigens present in cryostat sections of rat organs ( liver , kidney and stomach ) .
	manualset3
133283	1	406745	5	NULL	NULL	0	NULL	Sera 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera from white-tailed deer from Minnesota and Iowa were tested for antibodies to N. caninum by four serologic tests including the indirect fluorescent antibody ( IFA ) test ( cut-off 1 : 25 ) , Neospora caninum agglutination test ( cut-off 1 : 25 ) , an enzyme-linked immunoabsorbent assay , and Western blot ( WB ) .
	manualset3
133285	2	406745	5	NULL	NULL	0	NULL	white-tailed deer	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera from white-tailed deer from Minnesota and Iowa were tested for antibodies to N. caninum by four serologic tests including the indirect fluorescent antibody ( IFA ) test ( cut-off 1 : 25 ) , Neospora caninum agglutination test ( cut-off 1 : 25 ) , an enzyme-linked immunoabsorbent assay , and Western blot ( WB ) .
	manualset3
133287	3	406745	5	NULL	NULL	0	NULL	Minnesota 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera from white-tailed deer from Minnesota and Iowa were tested for antibodies to N. caninum by four serologic tests including the indirect fluorescent antibody ( IFA ) test ( cut-off 1 : 25 ) , Neospora caninum agglutination test ( cut-off 1 : 25 ) , an enzyme-linked immunoabsorbent assay , and Western blot ( WB ) .
	manualset3
133289	4	406745	5	NULL	NULL	0	NULL	Iowa 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera from white-tailed deer from Minnesota and Iowa were tested for antibodies to N. caninum by four serologic tests including the indirect fluorescent antibody ( IFA ) test ( cut-off 1 : 25 ) , Neospora caninum agglutination test ( cut-off 1 : 25 ) , an enzyme-linked immunoabsorbent assay , and Western blot ( WB ) .
	manualset3
133290	5	406745	5	NULL	NULL	0	NULL	antibodies 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera from white-tailed deer from Minnesota and Iowa were tested for antibodies to N. caninum by four serologic tests including the indirect fluorescent antibody ( IFA ) test ( cut-off 1 : 25 ) , Neospora caninum agglutination test ( cut-off 1 : 25 ) , an enzyme-linked immunoabsorbent assay , and Western blot ( WB ) .
	manualset3
133294	6	406745	5	NULL	NULL	0	NULL	N. caninum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera from white-tailed deer from Minnesota and Iowa were tested for antibodies to N. caninum by four serologic tests including the indirect fluorescent antibody ( IFA ) test ( cut-off 1 : 25 ) , Neospora caninum agglutination test ( cut-off 1 : 25 ) , an enzyme-linked immunoabsorbent assay , and Western blot ( WB ) .
	manualset3
133296	7	406745	5	NULL	NULL	0	NULL	four 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera from white-tailed deer from Minnesota and Iowa were tested for antibodies to N. caninum by four serologic tests including the indirect fluorescent antibody ( IFA ) test ( cut-off 1 : 25 ) , Neospora caninum agglutination test ( cut-off 1 : 25 ) , an enzyme-linked immunoabsorbent assay , and Western blot ( WB ) .
	manualset3
133297	8	406745	5	NULL	NULL	0	NULL	serologic tests 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera from white-tailed deer from Minnesota and Iowa were tested for antibodies to N. caninum by four serologic tests including the indirect fluorescent antibody ( IFA ) test ( cut-off 1 : 25 ) , Neospora caninum agglutination test ( cut-off 1 : 25 ) , an enzyme-linked immunoabsorbent assay , and Western blot ( WB ) .
	manualset3
133299	9	406745	5	NULL	NULL	0	NULL	indirect fluorescent antibody ( IFA ) test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera from white-tailed deer from Minnesota and Iowa were tested for antibodies to N. caninum by four serologic tests including the indirect fluorescent antibody ( IFA ) test ( cut-off 1 : 25 ) , Neospora caninum agglutination test ( cut-off 1 : 25 ) , an enzyme-linked immunoabsorbent assay , and Western blot ( WB ) .
	manualset3
133302	10	406745	5	NULL	NULL	0	NULL	cut-off 1 : 25	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera from white-tailed deer from Minnesota and Iowa were tested for antibodies to N. caninum by four serologic tests including the indirect fluorescent antibody ( IFA ) test ( cut-off 1 : 25 ) , Neospora caninum agglutination test ( cut-off 1 : 25 ) , an enzyme-linked immunoabsorbent assay , and Western blot ( WB ) .
	manualset3
133304	11	406745	5	NULL	NULL	0	NULL	 Neospora caninum agglutination test 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera from white-tailed deer from Minnesota and Iowa were tested for antibodies to N. caninum by four serologic tests including the indirect fluorescent antibody ( IFA ) test ( cut-off 1 : 25 ) , Neospora caninum agglutination test ( cut-off 1 : 25 ) , an enzyme-linked immunoabsorbent assay , and Western blot ( WB ) .
	manualset3
133305	12	406745	5	NULL	NULL	0	NULL	cut-off 1 : 25 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera from white-tailed deer from Minnesota and Iowa were tested for antibodies to N. caninum by four serologic tests including the indirect fluorescent antibody ( IFA ) test ( cut-off 1 : 25 ) , Neospora caninum agglutination test ( cut-off 1 : 25 ) , an enzyme-linked immunoabsorbent assay , and Western blot ( WB ) .
	manualset3
133313	13	406745	5	NULL	NULL	0	NULL	enzyme-linked immunoabsorbent assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera from white-tailed deer from Minnesota and Iowa were tested for antibodies to N. caninum by four serologic tests including the indirect fluorescent antibody ( IFA ) test ( cut-off 1 : 25 ) , Neospora caninum agglutination test ( cut-off 1 : 25 ) , an enzyme-linked immunoabsorbent assay , and Western blot ( WB ) .
	manualset3
133314	14	406745	5	NULL	NULL	0	NULL	Western blot ( WB )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera from white-tailed deer from Minnesota and Iowa were tested for antibodies to N. caninum by four serologic tests including the indirect fluorescent antibody ( IFA ) test ( cut-off 1 : 25 ) , Neospora caninum agglutination test ( cut-off 1 : 25 ) , an enzyme-linked immunoabsorbent assay , and Western blot ( WB ) .
	manualset3
133320	1	406746	5	NULL	NULL	0	NULL	strategy 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A new strategy is described for the assembly of large polypeptides on a solid support that utilizes a highly stable safety catch acid-labile linker .
	manualset3
133322	2	406746	5	NULL	NULL	0	NULL	assembly 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A new strategy is described for the assembly of large polypeptides on a solid support that utilizes a highly stable safety catch acid-labile linker .
	manualset3
133353	3	406746	5	NULL	NULL	0	NULL	large polypeptides 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	A new strategy is described for the assembly of large polypeptides on a solid support that utilizes a highly stable safety catch acid-labile linker .
	manualset3
133354	4	406746	5	NULL	NULL	0	NULL	solid support 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A new strategy is described for the assembly of large polypeptides on a solid support that utilizes a highly stable safety catch acid-labile linker .
	manualset3
133368	5	406746	5	NULL	NULL	0	NULL	highly stable safety catch acid-labile linker	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A new strategy is described for the assembly of large polypeptides on a solid support that utilizes a highly stable safety catch acid-labile linker .
	manualset3
133369	1	406747	5	NULL	NULL	0	NULL	Sera 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera obtained prior to , during and after the excretion of spirochetes were tested for antibodies in routine serology tests for leptospirosis and syphilis .
	manualset3
133373	2	406747	5	NULL	NULL	0	NULL	excretion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera obtained prior to , during and after the excretion of spirochetes were tested for antibodies in routine serology tests for leptospirosis and syphilis .
	manualset3
133380	3	406747	5	NULL	NULL	0	NULL	spirochetes 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera obtained prior to , during and after the excretion of spirochetes were tested for antibodies in routine serology tests for leptospirosis and syphilis .
	manualset3
133382	4	406747	5	NULL	NULL	0	NULL	antibodies 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera obtained prior to , during and after the excretion of spirochetes were tested for antibodies in routine serology tests for leptospirosis and syphilis .
	manualset3
133384	5	406747	5	NULL	NULL	0	NULL	routine serology tests 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera obtained prior to , during and after the excretion of spirochetes were tested for antibodies in routine serology tests for leptospirosis and syphilis .
	manualset3
133385	6	406747	5	NULL	NULL	0	NULL	leptospirosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera obtained prior to , during and after the excretion of spirochetes were tested for antibodies in routine serology tests for leptospirosis and syphilis .
	manualset3
133386	7	406747	5	NULL	NULL	0	NULL	syphilis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Sera obtained prior to , during and after the excretion of spirochetes were tested for antibodies in routine serology tests for leptospirosis and syphilis .
	manualset3
133387	1	406748	5	NULL	NULL	0	NULL	Serial blood collections	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Serial blood collections at 3-h intervals from 35 patients with acute myocardial infarction were examined .
	manualset3
133388	2	406748	5	NULL	NULL	0	NULL	 3-h intervals	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Serial blood collections at 3-h intervals from 35 patients with acute myocardial infarction were examined .
	manualset3
133389	3	406748	5	NULL	NULL	0	NULL	35 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Serial blood collections at 3-h intervals from 35 patients with acute myocardial infarction were examined .
	manualset3
133390	4	406748	5	NULL	NULL	0	NULL	acute myocardial infarction 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serial blood collections at 3-h intervals from 35 patients with acute myocardial infarction were examined .
	manualset3
133391	1	406749	5	NULL	NULL	0	NULL	Serial blood samples 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Serial blood samples were taken for up to two hours after the ingestion of a standard mixed meal ( 450 kcal ) and these showed a significant glucose intolerance , a reduced and delayed insulin response , and a reduced release of gastric inhibitory polypeptide , as compared with the controls .
	manualset3
133393	2	406749	5	NULL	NULL	0	NULL	two hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Serial blood samples were taken for up to two hours after the ingestion of a standard mixed meal ( 450 kcal ) and these showed a significant glucose intolerance , a reduced and delayed insulin response , and a reduced release of gastric inhibitory polypeptide , as compared with the controls .
	manualset3
133395	3	406749	5	NULL	NULL	0	NULL	ingestion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Serial blood samples were taken for up to two hours after the ingestion of a standard mixed meal ( 450 kcal ) and these showed a significant glucose intolerance , a reduced and delayed insulin response , and a reduced release of gastric inhibitory polypeptide , as compared with the controls .
	manualset3
133396	4	406749	5	NULL	NULL	0	NULL	standard mixed meal	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Serial blood samples were taken for up to two hours after the ingestion of a standard mixed meal ( 450 kcal ) and these showed a significant glucose intolerance , a reduced and delayed insulin response , and a reduced release of gastric inhibitory polypeptide , as compared with the controls .
	manualset3
133397	5	406749	5	NULL	NULL	0	NULL	450 kcal	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Serial blood samples were taken for up to two hours after the ingestion of a standard mixed meal ( 450 kcal ) and these showed a significant glucose intolerance , a reduced and delayed insulin response , and a reduced release of gastric inhibitory polypeptide , as compared with the controls .
	manualset3
133399	6	406749	5	NULL	NULL	0	NULL	significant glucose intolerance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serial blood samples were taken for up to two hours after the ingestion of a standard mixed meal ( 450 kcal ) and these showed a significant glucose intolerance , a reduced and delayed insulin response , and a reduced release of gastric inhibitory polypeptide , as compared with the controls .
	manualset3
133401	7	406749	5	NULL	NULL	0	NULL	reduced and delayed insulin response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serial blood samples were taken for up to two hours after the ingestion of a standard mixed meal ( 450 kcal ) and these showed a significant glucose intolerance , a reduced and delayed insulin response , and a reduced release of gastric inhibitory polypeptide , as compared with the controls .
	manualset3
133403	8	406749	5	NULL	NULL	0	NULL	reduced release of gastric inhibitory polypeptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Serial blood samples were taken for up to two hours after the ingestion of a standard mixed meal ( 450 kcal ) and these showed a significant glucose intolerance , a reduced and delayed insulin response , and a reduced release of gastric inhibitory polypeptide , as compared with the controls .
	manualset3
133404	9	406749	5	NULL	NULL	0	NULL	controls 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Serial blood samples were taken for up to two hours after the ingestion of a standard mixed meal ( 450 kcal ) and these showed a significant glucose intolerance , a reduced and delayed insulin response , and a reduced release of gastric inhibitory polypeptide , as compared with the controls .
	manualset3
133405	1	406750	5	NULL	NULL	0	NULL	Serial study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serial study of C reactive protein concentrations in cardiac allograft recipients .
	manualset3
133406	2	406750	5	NULL	NULL	0	NULL	C reactive protein concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serial study of C reactive protein concentrations in cardiac allograft recipients .
	manualset3
133407	3	406750	5	NULL	NULL	0	NULL	cardiac allograft recipients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Serial study of C reactive protein concentrations in cardiac allograft recipients .
	manualset3
133408	1	406751	5	NULL	NULL	0	NULL	Serine 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Serine , glycine , and cysteine were better incorporated than alanine or aspartate , whereas an excess of nonradioactive serine depressed the incorporation of labeled cysteine , glycine , and pyruvate .
	manualset3
133409	2	406751	5	NULL	NULL	0	NULL	glycine 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Serine , glycine , and cysteine were better incorporated than alanine or aspartate , whereas an excess of nonradioactive serine depressed the incorporation of labeled cysteine , glycine , and pyruvate .
	manualset3
133410	3	406751	5	NULL	NULL	0	NULL	cysteine 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Serine , glycine , and cysteine were better incorporated than alanine or aspartate , whereas an excess of nonradioactive serine depressed the incorporation of labeled cysteine , glycine , and pyruvate .
	manualset3
133411	4	406751	5	NULL	NULL	0	NULL	alanine 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Serine , glycine , and cysteine were better incorporated than alanine or aspartate , whereas an excess of nonradioactive serine depressed the incorporation of labeled cysteine , glycine , and pyruvate .
	manualset3
133412	5	406751	5	NULL	NULL	0	NULL	aspartate 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Serine , glycine , and cysteine were better incorporated than alanine or aspartate , whereas an excess of nonradioactive serine depressed the incorporation of labeled cysteine , glycine , and pyruvate .
	manualset3
133413	6	406751	5	NULL	NULL	0	NULL	nonradioactive serine 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Serine , glycine , and cysteine were better incorporated than alanine or aspartate , whereas an excess of nonradioactive serine depressed the incorporation of labeled cysteine , glycine , and pyruvate .
	manualset3
133414	7	406751	5	NULL	NULL	0	NULL	incorporation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Serine , glycine , and cysteine were better incorporated than alanine or aspartate , whereas an excess of nonradioactive serine depressed the incorporation of labeled cysteine , glycine , and pyruvate .
	manualset3
133415	8	406751	5	NULL	NULL	0	NULL	labeled cysteine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Serine , glycine , and cysteine were better incorporated than alanine or aspartate , whereas an excess of nonradioactive serine depressed the incorporation of labeled cysteine , glycine , and pyruvate .
	manualset3
133416	9	406751	5	NULL	NULL	0	NULL	glycine 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Serine , glycine , and cysteine were better incorporated than alanine or aspartate , whereas an excess of nonradioactive serine depressed the incorporation of labeled cysteine , glycine , and pyruvate .
	manualset3
133417	10	406751	5	NULL	NULL	0	NULL	pyruvate 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Serine , glycine , and cysteine were better incorporated than alanine or aspartate , whereas an excess of nonradioactive serine depressed the incorporation of labeled cysteine , glycine , and pyruvate .
	manualset3
133418	1	406752	5	NULL	NULL	0	NULL	 side-effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serious and newly detected side-effects after marketing were pseudomembranous colitis and melena , one case each .
	manualset3
133419	2	406752	5	NULL	NULL	0	NULL	marketing 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Serious and newly detected side-effects after marketing were pseudomembranous colitis and melena , one case each .
	manualset3
133420	3	406752	5	NULL	NULL	0	NULL	pseudomembranous colitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serious and newly detected side-effects after marketing were pseudomembranous colitis and melena , one case each .
	manualset3
133421	4	406752	5	NULL	NULL	0	NULL	melena 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serious and newly detected side-effects after marketing were pseudomembranous colitis and melena , one case each .
	manualset3
133422	5	406752	5	NULL	NULL	NULL	NULL	one case 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Serious and newly detected side-effects after marketing were pseudomembranous colitis and melena , one case each .
	manualset3
133423	1	406753	5	NULL	NULL	0	NULL	Serious poisonings 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serious poisonings among older adults : a study of hospitalization and mortality rates in Massachusetts 1983-85 .
	manualset3
133424	2	406753	5	NULL	NULL	0	NULL	older adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Serious poisonings among older adults : a study of hospitalization and mortality rates in Massachusetts 1983-85 .
	manualset3
133425	3	406753	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serious poisonings among older adults : a study of hospitalization and mortality rates in Massachusetts 1983-85 .
	manualset3
133426	4	406753	5	NULL	NULL	0	NULL	hospitalization 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Serious poisonings among older adults : a study of hospitalization and mortality rates in Massachusetts 1983-85 .
	manualset3
133427	5	406753	5	NULL	NULL	0	NULL	mortality rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serious poisonings among older adults : a study of hospitalization and mortality rates in Massachusetts 1983-85 .
	manualset3
133428	6	406753	5	NULL	NULL	0	NULL	Massachusetts 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Serious poisonings among older adults : a study of hospitalization and mortality rates in Massachusetts 1983-85 .
	manualset3
133429	7	406753	5	NULL	NULL	0	NULL	1983-85	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Serious poisonings among older adults : a study of hospitalization and mortality rates in Massachusetts 1983-85 .
	manualset3
133430	1	406754	5	NULL	NULL	0	NULL	Seroconversion rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Seroconversion rates to Edmonston Zagreb or AIK-C vaccines at 6 months of age were generally similar to those to Schwarz vaccine at 9 months of age , but antibody levels were lower after vaccination below 9 months of age .
	manualset3
133431	2	406754	5	NULL	NULL	0	NULL	Edmonston Zagreb or AIK-C vaccines	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Seroconversion rates to Edmonston Zagreb or AIK-C vaccines at 6 months of age were generally similar to those to Schwarz vaccine at 9 months of age , but antibody levels were lower after vaccination below 9 months of age .
	manualset3
133432	3	406754	5	NULL	NULL	0	NULL	6 months	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Seroconversion rates to Edmonston Zagreb or AIK-C vaccines at 6 months of age were generally similar to those to Schwarz vaccine at 9 months of age , but antibody levels were lower after vaccination below 9 months of age .
	manualset3
133433	4	406754	5	NULL	NULL	0	NULL	age 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Seroconversion rates to Edmonston Zagreb or AIK-C vaccines at 6 months of age were generally similar to those to Schwarz vaccine at 9 months of age , but antibody levels were lower after vaccination below 9 months of age .
	manualset3
133434	5	406754	5	NULL	NULL	0	NULL	Schwarz vaccine	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Seroconversion rates to Edmonston Zagreb or AIK-C vaccines at 6 months of age were generally similar to those to Schwarz vaccine at 9 months of age , but antibody levels were lower after vaccination below 9 months of age .
	manualset3
133435	6	406754	5	NULL	NULL	0	NULL	9 months 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Seroconversion rates to Edmonston Zagreb or AIK-C vaccines at 6 months of age were generally similar to those to Schwarz vaccine at 9 months of age , but antibody levels were lower after vaccination below 9 months of age .
	manualset3
133436	7	406754	5	NULL	NULL	0	NULL	age	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Seroconversion rates to Edmonston Zagreb or AIK-C vaccines at 6 months of age were generally similar to those to Schwarz vaccine at 9 months of age , but antibody levels were lower after vaccination below 9 months of age .
	manualset3
133437	8	406754	5	NULL	NULL	0	NULL	antibody levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Seroconversion rates to Edmonston Zagreb or AIK-C vaccines at 6 months of age were generally similar to those to Schwarz vaccine at 9 months of age , but antibody levels were lower after vaccination below 9 months of age .
	manualset3
133438	9	406754	5	NULL	NULL	0	NULL	vaccination 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Seroconversion rates to Edmonston Zagreb or AIK-C vaccines at 6 months of age were generally similar to those to Schwarz vaccine at 9 months of age , but antibody levels were lower after vaccination below 9 months of age .
	manualset3
133439	10	406754	5	NULL	NULL	0	NULL	9 months	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Seroconversion rates to Edmonston Zagreb or AIK-C vaccines at 6 months of age were generally similar to those to Schwarz vaccine at 9 months of age , but antibody levels were lower after vaccination below 9 months of age .
	manualset3
133440	11	406754	5	NULL	NULL	0	NULL	age 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Seroconversion rates to Edmonston Zagreb or AIK-C vaccines at 6 months of age were generally similar to those to Schwarz vaccine at 9 months of age , but antibody levels were lower after vaccination below 9 months of age .
	manualset3
133441	1	406755	5	NULL	NULL	0	NULL	new technique 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A new technique for estimating preference of habitat characteristics , applicable when there are multiple individual observations , is proposed .
	manualset3
133442	2	406755	5	NULL	NULL	0	NULL	preference 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A new technique for estimating preference of habitat characteristics , applicable when there are multiple individual observations , is proposed .
	manualset3
133443	3	406755	5	NULL	NULL	0	NULL	habitat characteristics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new technique for estimating preference of habitat characteristics , applicable when there are multiple individual observations , is proposed .
	manualset3
133444	4	406755	5	NULL	NULL	0	NULL	multiple individual observations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A new technique for estimating preference of habitat characteristics , applicable when there are multiple individual observations , is proposed .
	manualset3
133445	1	406756	5	NULL	NULL	0	NULL	Seroconversion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Seroconversion to SPf66 by enzyme-linked immunosorbent assay occurred in 76 % of volunteers receiving two or three doses .
	manualset3
133446	2	406756	5	NULL	NULL	0	NULL	SPf66 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Seroconversion to SPf66 by enzyme-linked immunosorbent assay occurred in 76 % of volunteers receiving two or three doses .
	manualset3
133447	3	406756	5	NULL	NULL	0	NULL	enzyme-linked immunosorbent assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Seroconversion to SPf66 by enzyme-linked immunosorbent assay occurred in 76 % of volunteers receiving two or three doses .
	manualset3
133448	4	406756	5	NULL	NULL	0	NULL	 76 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Seroconversion to SPf66 by enzyme-linked immunosorbent assay occurred in 76 % of volunteers receiving two or three doses .
	manualset3
133449	5	406756	5	NULL	NULL	0	NULL	volunteers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Seroconversion to SPf66 by enzyme-linked immunosorbent assay occurred in 76 % of volunteers receiving two or three doses .
	manualset3
133450	6	406756	5	NULL	NULL	0	NULL	two or three doses 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Seroconversion to SPf66 by enzyme-linked immunosorbent assay occurred in 76 % of volunteers receiving two or three doses .
	manualset3
133451	1	406757	5	NULL	NULL	0	NULL	Serodiagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Serodiagnosis of swine pleuropneumonia due to Actinobacillus pleuropneumoniae serotypes 7 and 4 using long-chain lipopolysaccharides .
	manualset3
133452	2	406757	5	NULL	NULL	0	NULL	swine pleuropneumonia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Serodiagnosis of swine pleuropneumonia due to Actinobacillus pleuropneumoniae serotypes 7 and 4 using long-chain lipopolysaccharides .
	manualset3
133453	3	406757	5	NULL	NULL	0	NULL	Actinobacillus pleuropneumoniae serotype 7	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Serodiagnosis of swine pleuropneumonia due to Actinobacillus pleuropneumoniae serotypes 7 and 4 using long-chain lipopolysaccharides .
	manualset3
133454	4	406757	5	NULL	NULL	0	NULL	Actinobacillus pleuropneumoniae serotype 4	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Serodiagnosis of swine pleuropneumonia due to Actinobacillus pleuropneumoniae serotypes 7 and 4 using long-chain lipopolysaccharides .
	manualset3
133455	5	406757	5	NULL	NULL	0	NULL	long-chain lipopolysaccharides	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Serodiagnosis of swine pleuropneumonia due to Actinobacillus pleuropneumoniae serotypes 7 and 4 using long-chain lipopolysaccharides .
	manualset3
133456	1	406758	5	NULL	NULL	0	NULL	Serologic response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serologic response to Helicobacter pylori among children and teenagers in northern Chile .
	manualset3
133457	2	406758	5	NULL	NULL	0	NULL	Helicobacter pylori	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Serologic response to Helicobacter pylori among children and teenagers in northern Chile .
	manualset3
133458	3	406758	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Serologic response to Helicobacter pylori among children and teenagers in northern Chile .
	manualset3
133459	4	406758	5	NULL	NULL	0	NULL	teenagers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Serologic response to Helicobacter pylori among children and teenagers in northern Chile .
	manualset3
133460	5	406758	5	NULL	NULL	0	NULL	northern Chile	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Serologic response to Helicobacter pylori among children and teenagers in northern Chile .
	manualset3
133461	1	406759	5	NULL	NULL	0	NULL	Serological diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serological diagnosis of dengue by an ELISA inhibition method ( EIM ) .
	manualset3
133462	2	406759	5	NULL	NULL	0	NULL	dengue 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Serological diagnosis of dengue by an ELISA inhibition method ( EIM ) .
	manualset3
133463	3	406759	5	NULL	NULL	0	NULL	ELISA inhibition method ( EIM )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serological diagnosis of dengue by an ELISA inhibition method ( EIM ) .
	manualset3
133464	1	406760	5	NULL	NULL	0	NULL	Serological immune response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serological immune response to H. pylori in gastric cancer , non-gastric cancer and outpatients seems different both quantitatively and qualitatively ; serology was more reliable than histology in detection of H. pylori in gastric cancer .
	manualset3
133465	2	406760	5	NULL	NULL	0	NULL	H. pylori	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Serological immune response to H. pylori in gastric cancer , non-gastric cancer and outpatients seems different both quantitatively and qualitatively ; serology was more reliable than histology in detection of H. pylori in gastric cancer .
	manualset3
133466	3	406760	5	NULL	NULL	0	NULL	gastric cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Serological immune response to H. pylori in gastric cancer , non-gastric cancer and outpatients seems different both quantitatively and qualitatively ; serology was more reliable than histology in detection of H. pylori in gastric cancer .
	manualset3
133467	4	406760	5	NULL	NULL	0	NULL	non-gastric cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Serological immune response to H. pylori in gastric cancer , non-gastric cancer and outpatients seems different both quantitatively and qualitatively ; serology was more reliable than histology in detection of H. pylori in gastric cancer .
	manualset3
133468	5	406760	5	NULL	NULL	0	NULL	outpatients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Serological immune response to H. pylori in gastric cancer , non-gastric cancer and outpatients seems different both quantitatively and qualitatively ; serology was more reliable than histology in detection of H. pylori in gastric cancer .
	manualset3
133469	6	406760	5	NULL	NULL	0	NULL	serology 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Serological immune response to H. pylori in gastric cancer , non-gastric cancer and outpatients seems different both quantitatively and qualitatively ; serology was more reliable than histology in detection of H. pylori in gastric cancer .
	manualset3
133470	7	406760	5	NULL	NULL	0	NULL	histology 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Serological immune response to H. pylori in gastric cancer , non-gastric cancer and outpatients seems different both quantitatively and qualitatively ; serology was more reliable than histology in detection of H. pylori in gastric cancer .
	manualset3
133471	8	406760	5	NULL	NULL	0	NULL	detection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serological immune response to H. pylori in gastric cancer , non-gastric cancer and outpatients seems different both quantitatively and qualitatively ; serology was more reliable than histology in detection of H. pylori in gastric cancer .
	manualset3
133472	9	406760	5	NULL	NULL	0	NULL	H. pylori	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Serological immune response to H. pylori in gastric cancer , non-gastric cancer and outpatients seems different both quantitatively and qualitatively ; serology was more reliable than histology in detection of H. pylori in gastric cancer .
	manualset3
133473	10	406760	5	NULL	NULL	0	NULL	gastric cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Serological immune response to H. pylori in gastric cancer , non-gastric cancer and outpatients seems different both quantitatively and qualitatively ; serology was more reliable than histology in detection of H. pylori in gastric cancer .
	manualset3
133474	1	406761	5	NULL	NULL	NULL	NULL	new type of familial pHPT	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A new type of familial pHPT was recently discovered .
	manualset3
133475	1	406762	5	NULL	NULL	0	NULL	Serological parameters	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serological parameters of bone and fibrous tissue turnover were demonstrated to monitor the course of fracture healing .
	manualset3
133476	2	406762	5	NULL	NULL	NULL	NULL	bone tissue turnover	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Serological parameters of bone and fibrous tissue turnover were demonstrated to monitor the course of fracture healing .
	manualset3
133477	3	406762	5	NULL	NULL	0	NULL	fibrous tissue turnover	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Serological parameters of bone and fibrous tissue turnover were demonstrated to monitor the course of fracture healing .
	manualset3
133479	5	406762	5	NULL	NULL	0	NULL	course 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Serological parameters of bone and fibrous tissue turnover were demonstrated to monitor the course of fracture healing .
	manualset3
133480	6	406762	5	NULL	NULL	0	NULL	fracture healing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serological parameters of bone and fibrous tissue turnover were demonstrated to monitor the course of fracture healing .
	manualset3
133481	1	406763	5	NULL	NULL	0	NULL	Serotonergic modulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Serotonergic modulation can be mimicked by perfusion with membrane-permeable analogs of either adenine ( cAMP ) or guanine ( cGMP ) cyclic nucleotides , and is prolonged in the presence of phosphodiesterase inhibitors .
	manualset3
133482	2	406763	5	NULL	NULL	0	NULL	perfusion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Serotonergic modulation can be mimicked by perfusion with membrane-permeable analogs of either adenine ( cAMP ) or guanine ( cGMP ) cyclic nucleotides , and is prolonged in the presence of phosphodiesterase inhibitors .
	manualset3
133483	3	406763	5	NULL	NULL	0	NULL	membrane-permeable analogs of adenine ( cAMP ) cyclic nucleotides	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Serotonergic modulation can be mimicked by perfusion with membrane-permeable analogs of either adenine ( cAMP ) or guanine ( cGMP ) cyclic nucleotides , and is prolonged in the presence of phosphodiesterase inhibitors .
	manualset3
133484	4	406763	5	NULL	NULL	0	NULL	membrane-permeable analogs of guanine ( cGMP ) cyclic nucleotides	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Serotonergic modulation can be mimicked by perfusion with membrane-permeable analogs of either adenine ( cAMP ) or guanine ( cGMP ) cyclic nucleotides , and is prolonged in the presence of phosphodiesterase inhibitors .
	manualset3
133485	5	406763	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Serotonergic modulation can be mimicked by perfusion with membrane-permeable analogs of either adenine ( cAMP ) or guanine ( cGMP ) cyclic nucleotides , and is prolonged in the presence of phosphodiesterase inhibitors .
	manualset3
133486	6	406763	5	NULL	NULL	0	NULL	phosphodiesterase inhibitors	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Serotonergic modulation can be mimicked by perfusion with membrane-permeable analogs of either adenine ( cAMP ) or guanine ( cGMP ) cyclic nucleotides , and is prolonged in the presence of phosphodiesterase inhibitors .
	manualset3
133487	1	406764	5	NULL	NULL	0	NULL	Serotonin Syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Serotonin Syndrome : SSRIs , SNRIs , Triptans , and Current Clinical Practice .
	manualset3
133488	2	406764	5	NULL	NULL	0	NULL	SSRIs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Serotonin Syndrome : SSRIs , SNRIs , Triptans , and Current Clinical Practice .
	manualset3
133489	3	406764	5	NULL	NULL	0	NULL	SNRIs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Serotonin Syndrome : SSRIs , SNRIs , Triptans , and Current Clinical Practice .
	manualset3
133490	4	406764	5	NULL	NULL	0	NULL	Triptans 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Serotonin Syndrome : SSRIs , SNRIs , Triptans , and Current Clinical Practice .
	manualset3
133491	5	406764	5	NULL	NULL	0	NULL	Current Clinical Practice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Serotonin Syndrome : SSRIs , SNRIs , Triptans , and Current Clinical Practice .
	manualset3
133492	1	406765	5	NULL	NULL	0	NULL	Serotoninergic and peptidergic nerve elements	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serotoninergic and peptidergic nerve elements in the protoscolex of Echinococcus granulosus ( Cestoda , Cyclophyllidea ) .
	manualset3
133493	2	406765	5	NULL	NULL	0	NULL	protoscolex 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Serotoninergic and peptidergic nerve elements in the protoscolex of Echinococcus granulosus ( Cestoda , Cyclophyllidea ) .
	manualset3
133494	3	406765	5	NULL	NULL	0	NULL	Echinococcus granulosus ( Cestoda , Cyclophyllidea )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Serotoninergic and peptidergic nerve elements in the protoscolex of Echinococcus granulosus ( Cestoda , Cyclophyllidea ) .
	manualset3
133495	1	406766	5	NULL	NULL	0	NULL	Serum-ferritin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum-ferritin in diagnosis of hemochromatosis .
	manualset3
133496	2	406766	5	NULL	NULL	0	NULL	diagnosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum-ferritin in diagnosis of hemochromatosis .
	manualset3
133497	3	406766	5	NULL	NULL	0	NULL	hemochromatosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum-ferritin in diagnosis of hemochromatosis .
	manualset3
133498	1	406767	5	NULL	NULL	0	NULL	new type of lambda6-sulfanenitrile	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A new type of lambda6-sulfanenitrile with an SN triple bond at both ends , Ph2S ( = N - ( Ph2 ) S ( triple bond ) N ) 2 ( 5 ) , was prepared in excellent yield from the one-pot synthesis of diphenylsulfimide ( Ph2SNH ) with fluoro ( diphenyl ) - lambda6-sulfanenitrile ( Ph2FSN ) in the presence of 1 , 8-diazabicyclo ( 5.4.0 ) undec-7-ene .
	manualset3
133499	2	406767	5	NULL	NULL	0	NULL	SN triple bond	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A new type of lambda6-sulfanenitrile with an SN triple bond at both ends , Ph2S ( = N - ( Ph2 ) S ( triple bond ) N ) 2 ( 5 ) , was prepared in excellent yield from the one-pot synthesis of diphenylsulfimide ( Ph2SNH ) with fluoro ( diphenyl ) - lambda6-sulfanenitrile ( Ph2FSN ) in the presence of 1 , 8-diazabicyclo ( 5.4.0 ) undec-7-ene .
	manualset3
133500	3	406767	5	NULL	NULL	0	NULL	Ph2S ( = N - ( Ph2 ) S ( triple bond ) N ) 2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A new type of lambda6-sulfanenitrile with an SN triple bond at both ends , Ph2S ( = N - ( Ph2 ) S ( triple bond ) N ) 2 ( 5 ) , was prepared in excellent yield from the one-pot synthesis of diphenylsulfimide ( Ph2SNH ) with fluoro ( diphenyl ) - lambda6-sulfanenitrile ( Ph2FSN ) in the presence of 1 , 8-diazabicyclo ( 5.4.0 ) undec-7-ene .
	manualset3
133501	4	406767	5	NULL	NULL	0	NULL	yield 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new type of lambda6-sulfanenitrile with an SN triple bond at both ends , Ph2S ( = N - ( Ph2 ) S ( triple bond ) N ) 2 ( 5 ) , was prepared in excellent yield from the one-pot synthesis of diphenylsulfimide ( Ph2SNH ) with fluoro ( diphenyl ) - lambda6-sulfanenitrile ( Ph2FSN ) in the presence of 1 , 8-diazabicyclo ( 5.4.0 ) undec-7-ene .
	manualset3
133502	5	406767	5	NULL	NULL	0	NULL	 one-pot synthesis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new type of lambda6-sulfanenitrile with an SN triple bond at both ends , Ph2S ( = N - ( Ph2 ) S ( triple bond ) N ) 2 ( 5 ) , was prepared in excellent yield from the one-pot synthesis of diphenylsulfimide ( Ph2SNH ) with fluoro ( diphenyl ) - lambda6-sulfanenitrile ( Ph2FSN ) in the presence of 1 , 8-diazabicyclo ( 5.4.0 ) undec-7-ene .
	manualset3
133503	6	406767	5	NULL	NULL	0	NULL	diphenylsulfimide ( Ph2SNH ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A new type of lambda6-sulfanenitrile with an SN triple bond at both ends , Ph2S ( = N - ( Ph2 ) S ( triple bond ) N ) 2 ( 5 ) , was prepared in excellent yield from the one-pot synthesis of diphenylsulfimide ( Ph2SNH ) with fluoro ( diphenyl ) - lambda6-sulfanenitrile ( Ph2FSN ) in the presence of 1 , 8-diazabicyclo ( 5.4.0 ) undec-7-ene .
	manualset3
133504	7	406767	5	NULL	NULL	0	NULL	fluoro ( diphenyl ) - lambda6-sulfanenitrile ( Ph2FSN )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A new type of lambda6-sulfanenitrile with an SN triple bond at both ends , Ph2S ( = N - ( Ph2 ) S ( triple bond ) N ) 2 ( 5 ) , was prepared in excellent yield from the one-pot synthesis of diphenylsulfimide ( Ph2SNH ) with fluoro ( diphenyl ) - lambda6-sulfanenitrile ( Ph2FSN ) in the presence of 1 , 8-diazabicyclo ( 5.4.0 ) undec-7-ene .
	manualset3
133505	8	406767	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A new type of lambda6-sulfanenitrile with an SN triple bond at both ends , Ph2S ( = N - ( Ph2 ) S ( triple bond ) N ) 2 ( 5 ) , was prepared in excellent yield from the one-pot synthesis of diphenylsulfimide ( Ph2SNH ) with fluoro ( diphenyl ) - lambda6-sulfanenitrile ( Ph2FSN ) in the presence of 1 , 8-diazabicyclo ( 5.4.0 ) undec-7-ene .
	manualset3
133506	9	406767	5	NULL	NULL	0	NULL	1 , 8-diazabicyclo ( 5.4.0 ) undec-7-ene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A new type of lambda6-sulfanenitrile with an SN triple bond at both ends , Ph2S ( = N - ( Ph2 ) S ( triple bond ) N ) 2 ( 5 ) , was prepared in excellent yield from the one-pot synthesis of diphenylsulfimide ( Ph2SNH ) with fluoro ( diphenyl ) - lambda6-sulfanenitrile ( Ph2FSN ) in the presence of 1 , 8-diazabicyclo ( 5.4.0 ) undec-7-ene .
	manualset3
133507	1	406768	5	NULL	NULL	0	NULL	Serum 25-hydroxyvitamin D 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum 25-hydroxyvitamin D and depressive symptoms in older women and men .
	manualset3
133508	2	406768	5	NULL	NULL	0	NULL	depressive symptom	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum 25-hydroxyvitamin D and depressive symptoms in older women and men .
	manualset3
133509	3	406768	5	NULL	NULL	0	NULL	older women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum 25-hydroxyvitamin D and depressive symptoms in older women and men .
	manualset3
133510	4	406768	5	NULL	NULL	0	NULL	men 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum 25-hydroxyvitamin D and depressive symptoms in older women and men .
	manualset3
133511	1	406769	5	NULL	NULL	0	NULL	Serum 3-hydroxybutyrate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum 3-hydroxybutyrate , NEFA , triacylglycerols and glucose showed only slight changes in all groups vs. controls ; OE-treated rats showed lower cholesterol .
	manualset3
133512	2	406769	5	NULL	NULL	0	NULL	NEFA	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum 3-hydroxybutyrate , NEFA , triacylglycerols and glucose showed only slight changes in all groups vs. controls ; OE-treated rats showed lower cholesterol .
	manualset3
133513	3	406769	5	NULL	NULL	0	NULL	triacylglycerols 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum 3-hydroxybutyrate , NEFA , triacylglycerols and glucose showed only slight changes in all groups vs. controls ; OE-treated rats showed lower cholesterol .
	manualset3
133514	4	406769	5	NULL	NULL	0	NULL	glucose 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum 3-hydroxybutyrate , NEFA , triacylglycerols and glucose showed only slight changes in all groups vs. controls ; OE-treated rats showed lower cholesterol .
	manualset3
133515	5	406769	5	NULL	NULL	0	NULL	groups 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum 3-hydroxybutyrate , NEFA , triacylglycerols and glucose showed only slight changes in all groups vs. controls ; OE-treated rats showed lower cholesterol .
	manualset3
133516	6	406769	5	NULL	NULL	0	NULL	controls 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum 3-hydroxybutyrate , NEFA , triacylglycerols and glucose showed only slight changes in all groups vs. controls ; OE-treated rats showed lower cholesterol .
	manualset3
133517	7	406769	5	NULL	NULL	0	NULL	OE-treated rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum 3-hydroxybutyrate , NEFA , triacylglycerols and glucose showed only slight changes in all groups vs. controls ; OE-treated rats showed lower cholesterol .
	manualset3
133518	8	406769	5	NULL	NULL	0	NULL	lower cholesterol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum 3-hydroxybutyrate , NEFA , triacylglycerols and glucose showed only slight changes in all groups vs. controls ; OE-treated rats showed lower cholesterol .
	manualset3
134876	9	406769	5	NULL	NULL	0	NULL	changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum 3-hydroxybutyrate , NEFA , triacylglycerols and glucose showed only slight changes in all groups vs. controls ; OE-treated rats showed lower cholesterol .
	manualset3
133519	1	406770	5	NULL	NULL	0	NULL	Serum C4 concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum C4 concentrations were lower in the HIV Ab + patient group ( 33.9 + / - 10.1 versus 41.6 + / - 12.4 mg/dL , p = 0.043 ) .
	manualset3
133520	2	406770	5	NULL	NULL	0	NULL	HIV Ab + patient group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum C4 concentrations were lower in the HIV Ab + patient group ( 33.9 + / - 10.1 versus 41.6 + / - 12.4 mg/dL , p = 0.043 ) .
	manualset3
133521	3	406770	5	NULL	NULL	0	NULL	33.9 + / - 10.1 versus 41.6 + / - 12.4 mg/dL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum C4 concentrations were lower in the HIV Ab + patient group ( 33.9 + / - 10.1 versus 41.6 + / - 12.4 mg/dL , p = 0.043 ) .
	manualset3
133522	4	406770	5	NULL	NULL	0	NULL	p = 0.043	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum C4 concentrations were lower in the HIV Ab + patient group ( 33.9 + / - 10.1 versus 41.6 + / - 12.4 mg/dL , p = 0.043 ) .
	manualset3
133523	1	406771	5	NULL	NULL	0	NULL	Serum IgA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum IgA exerted a bacteriostatic effect in vitro on E. coli and P. aeruginosa , which increased in the presence of the iron-binding proteins lactoferrin and transferrin .
	manualset3
133524	2	406771	5	NULL	NULL	0	NULL	bacteriostatic effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum IgA exerted a bacteriostatic effect in vitro on E. coli and P. aeruginosa , which increased in the presence of the iron-binding proteins lactoferrin and transferrin .
	manualset3
133525	3	406771	5	NULL	NULL	0	NULL	 E. coli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum IgA exerted a bacteriostatic effect in vitro on E. coli and P. aeruginosa , which increased in the presence of the iron-binding proteins lactoferrin and transferrin .
	manualset3
133526	4	406771	5	NULL	NULL	0	NULL	P. aeruginosa	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum IgA exerted a bacteriostatic effect in vitro on E. coli and P. aeruginosa , which increased in the presence of the iron-binding proteins lactoferrin and transferrin .
	manualset3
133527	5	406771	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum IgA exerted a bacteriostatic effect in vitro on E. coli and P. aeruginosa , which increased in the presence of the iron-binding proteins lactoferrin and transferrin .
	manualset3
133528	6	406771	5	NULL	NULL	0	NULL	iron-binding protein lactoferrin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum IgA exerted a bacteriostatic effect in vitro on E. coli and P. aeruginosa , which increased in the presence of the iron-binding proteins lactoferrin and transferrin .
	manualset3
133529	7	406771	5	NULL	NULL	0	NULL	iron-binding protein transferrin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum IgA exerted a bacteriostatic effect in vitro on E. coli and P. aeruginosa , which increased in the presence of the iron-binding proteins lactoferrin and transferrin .
	manualset3
133530	1	406772	5	NULL	NULL	0	NULL	Serum IgE levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum IgE levels in cutaneous leishmaniasis by ELISA .
	manualset3
133531	2	406772	5	NULL	NULL	0	NULL	cutaneous leishmaniasis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum IgE levels in cutaneous leishmaniasis by ELISA .
	manualset3
133532	3	406772	5	NULL	NULL	0	NULL	ELISA 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum IgE levels in cutaneous leishmaniasis by ELISA .
	manualset3
133533	1	406773	5	NULL	NULL	0	NULL	Serum alanine aminotransferase levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum alanine aminotransferase levels were also increased but to a lesser degree in most patients .
	manualset3
133534	2	406773	5	NULL	NULL	0	NULL	lesser degree	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum alanine aminotransferase levels were also increased but to a lesser degree in most patients .
	manualset3
133535	3	406773	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum alanine aminotransferase levels were also increased but to a lesser degree in most patients .
	manualset3
133536	1	406774	5	NULL	NULL	0	NULL	Serum albumin level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum albumin level and nosocomial pneumonia in stroke patients .
	manualset3
133537	2	406774	5	NULL	NULL	0	NULL	nosocomial pneumonia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum albumin level and nosocomial pneumonia in stroke patients .
	manualset3
133538	3	406774	5	NULL	NULL	0	NULL	stroke patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum albumin level and nosocomial pneumonia in stroke patients .
	manualset3
133539	1	406775	5	NULL	NULL	0	NULL	Serum alkaline phosphatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum alkaline phosphatase , nucleotide pyrophosphatase , 5 ' - nucleotide and lipoprotein-X in cholestasis .
	manualset3
133540	2	406775	5	NULL	NULL	0	NULL	nucleotide pyrophosphatase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum alkaline phosphatase , nucleotide pyrophosphatase , 5 ' - nucleotide and lipoprotein-X in cholestasis .
	manualset3
133541	3	406775	5	NULL	NULL	0	NULL	 5 ' - nucleotide	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum alkaline phosphatase , nucleotide pyrophosphatase , 5 ' - nucleotide and lipoprotein-X in cholestasis .
	manualset3
133542	4	406775	5	NULL	NULL	0	NULL	lipoprotein-X	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum alkaline phosphatase , nucleotide pyrophosphatase , 5 ' - nucleotide and lipoprotein-X in cholestasis .
	manualset3
133543	5	406775	5	NULL	NULL	0	NULL	cholestasis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum alkaline phosphatase , nucleotide pyrophosphatase , 5 ' - nucleotide and lipoprotein-X in cholestasis .
	manualset3
133544	1	406776	5	NULL	NULL	NULL	NULL	variant of glucose-6-phosphate dehydrogenase deficiency hereditary hemolytic anemia , G6PD Cornell	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A new variant of glucose-6-phosphate dehydrogenase deficiency hereditary hemolytic anemia , G6PD Cornell : erythrocyte , leukocyte , and platelet studies .
	manualset3
133545	2	406776	5	NULL	NULL	0	NULL	erythrocyte studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new variant of glucose-6-phosphate dehydrogenase deficiency hereditary hemolytic anemia , G6PD Cornell : erythrocyte , leukocyte , and platelet studies .
	manualset3
133546	3	406776	5	NULL	NULL	0	NULL	leukocyte studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new variant of glucose-6-phosphate dehydrogenase deficiency hereditary hemolytic anemia , G6PD Cornell : erythrocyte , leukocyte , and platelet studies .
	manualset3
133547	4	406776	5	NULL	NULL	0	NULL	platelet studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new variant of glucose-6-phosphate dehydrogenase deficiency hereditary hemolytic anemia , G6PD Cornell : erythrocyte , leukocyte , and platelet studies .
	manualset3
133548	1	406777	5	NULL	NULL	0	NULL	Serum concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum and bile concentrations of GABA , 3H-GABA and 3H-metabolites of GABA were determined during the course of each GABA infusion period .
	manualset3
133549	2	406777	5	NULL	NULL	0	NULL	bile concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum and bile concentrations of GABA , 3H-GABA and 3H-metabolites of GABA were determined during the course of each GABA infusion period .
	manualset3
133550	3	406777	5	NULL	NULL	0	NULL	GABA 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum and bile concentrations of GABA , 3H-GABA and 3H-metabolites of GABA were determined during the course of each GABA infusion period .
	manualset3
133551	4	406777	5	NULL	NULL	0	NULL	 3H-GABA	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum and bile concentrations of GABA , 3H-GABA and 3H-metabolites of GABA were determined during the course of each GABA infusion period .
	manualset3
133552	5	406777	5	NULL	NULL	0	NULL	3H-metabolites of GABA	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum and bile concentrations of GABA , 3H-GABA and 3H-metabolites of GABA were determined during the course of each GABA infusion period .
	manualset3
133553	6	406777	5	NULL	NULL	0	NULL	course 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum and bile concentrations of GABA , 3H-GABA and 3H-metabolites of GABA were determined during the course of each GABA infusion period .
	manualset3
133554	7	406777	5	NULL	NULL	0	NULL	GABA infusion period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum and bile concentrations of GABA , 3H-GABA and 3H-metabolites of GABA were determined during the course of each GABA infusion period .
	manualset3
133555	1	406778	5	NULL	NULL	0	NULL	Serum level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum and urinary levels of alpha 1-microglobulin ( AM ) were measured in healthy volunteers and patients with varying degrees of renal insufficiency ( from mild impairment to functionally anephric patients ) .
	manualset3
133556	2	406778	5	NULL	NULL	0	NULL	urinary level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum and urinary levels of alpha 1-microglobulin ( AM ) were measured in healthy volunteers and patients with varying degrees of renal insufficiency ( from mild impairment to functionally anephric patients ) .
	manualset3
133557	3	406778	5	NULL	NULL	0	NULL	alpha 1-microglobulin ( AM ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum and urinary levels of alpha 1-microglobulin ( AM ) were measured in healthy volunteers and patients with varying degrees of renal insufficiency ( from mild impairment to functionally anephric patients ) .
	manualset3
133558	4	406778	5	NULL	NULL	0	NULL	healthy volunteers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum and urinary levels of alpha 1-microglobulin ( AM ) were measured in healthy volunteers and patients with varying degrees of renal insufficiency ( from mild impairment to functionally anephric patients ) .
	manualset3
133559	5	406778	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum and urinary levels of alpha 1-microglobulin ( AM ) were measured in healthy volunteers and patients with varying degrees of renal insufficiency ( from mild impairment to functionally anephric patients ) .
	manualset3
133560	6	406778	5	NULL	NULL	0	NULL	varying degrees	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum and urinary levels of alpha 1-microglobulin ( AM ) were measured in healthy volunteers and patients with varying degrees of renal insufficiency ( from mild impairment to functionally anephric patients ) .
	manualset3
133561	7	406778	5	NULL	NULL	0	NULL	renal insufficiency 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum and urinary levels of alpha 1-microglobulin ( AM ) were measured in healthy volunteers and patients with varying degrees of renal insufficiency ( from mild impairment to functionally anephric patients ) .
	manualset3
133562	8	406778	5	NULL	NULL	0	NULL	mild impairment 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum and urinary levels of alpha 1-microglobulin ( AM ) were measured in healthy volunteers and patients with varying degrees of renal insufficiency ( from mild impairment to functionally anephric patients ) .
	manualset3
133563	9	406778	5	NULL	NULL	0	NULL	functionally anephric patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum and urinary levels of alpha 1-microglobulin ( AM ) were measured in healthy volunteers and patients with varying degrees of renal insufficiency ( from mild impairment to functionally anephric patients ) .
	manualset3
133564	1	406779	5	NULL	NULL	0	NULL	Serum calcium level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum calcium and parathyroid hormone levels were decreased .
	manualset3
133565	2	406779	5	NULL	NULL	0	NULL	parathyroid hormone level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum calcium and parathyroid hormone levels were decreased .
	manualset3
133566	1	406780	5	NULL	NULL	0	NULL	Serum chemical analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum chemical analyses revealed profound hypernatremia and hyperchloremia .
	manualset3
133567	2	406780	5	NULL	NULL	0	NULL	hypernatremia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum chemical analyses revealed profound hypernatremia and hyperchloremia .
	manualset3
133568	3	406780	5	NULL	NULL	0	NULL	hyperchloremia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum chemical analyses revealed profound hypernatremia and hyperchloremia .
	manualset3
133768	1	406781	5	NULL	NULL	0	NULL	Serum concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum concentration of adiponectin and sICAM-1 did not correlate but sICAM-1 was independently , positively associated with sVCAM-1 ( p & lt ; 0.0001 ) and negatively with markers of insulin resistance and inflammation , namely atherogenic index log ( triglycerides/HDL-cholesterol ) ( p & lt ; 0.0001 ) , hs-CRP ( p & lt ; 0.001 ) and HOMA ( p & lt ; 0.05 ) .
	manualset3
133770	2	406781	5	NULL	NULL	0	NULL	adiponectin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum concentration of adiponectin and sICAM-1 did not correlate but sICAM-1 was independently , positively associated with sVCAM-1 ( p & lt ; 0.0001 ) and negatively with markers of insulin resistance and inflammation , namely atherogenic index log ( triglycerides/HDL-cholesterol ) ( p & lt ; 0.0001 ) , hs-CRP ( p & lt ; 0.001 ) and HOMA ( p & lt ; 0.05 ) .
	manualset3
133771	3	406781	5	NULL	NULL	0	NULL	 sICAM-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum concentration of adiponectin and sICAM-1 did not correlate but sICAM-1 was independently , positively associated with sVCAM-1 ( p & lt ; 0.0001 ) and negatively with markers of insulin resistance and inflammation , namely atherogenic index log ( triglycerides/HDL-cholesterol ) ( p & lt ; 0.0001 ) , hs-CRP ( p & lt ; 0.001 ) and HOMA ( p & lt ; 0.05 ) .
	manualset3
133776	5	406781	5	NULL	NULL	0	NULL	sICAM-1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum concentration of adiponectin and sICAM-1 did not correlate but sICAM-1 was independently , positively associated with sVCAM-1 ( p & lt ; 0.0001 ) and negatively with markers of insulin resistance and inflammation , namely atherogenic index log ( triglycerides/HDL-cholesterol ) ( p & lt ; 0.0001 ) , hs-CRP ( p & lt ; 0.001 ) and HOMA ( p & lt ; 0.05 ) .
	manualset3
133778	6	406781	5	NULL	NULL	0	NULL	 sVCAM-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum concentration of adiponectin and sICAM-1 did not correlate but sICAM-1 was independently , positively associated with sVCAM-1 ( p & lt ; 0.0001 ) and negatively with markers of insulin resistance and inflammation , namely atherogenic index log ( triglycerides/HDL-cholesterol ) ( p & lt ; 0.0001 ) , hs-CRP ( p & lt ; 0.001 ) and HOMA ( p & lt ; 0.05 ) .
	manualset3
133780	7	406781	5	NULL	NULL	0	NULL	 p & lt ; 0.0001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum concentration of adiponectin and sICAM-1 did not correlate but sICAM-1 was independently , positively associated with sVCAM-1 ( p & lt ; 0.0001 ) and negatively with markers of insulin resistance and inflammation , namely atherogenic index log ( triglycerides/HDL-cholesterol ) ( p & lt ; 0.0001 ) , hs-CRP ( p & lt ; 0.001 ) and HOMA ( p & lt ; 0.05 ) .
	manualset3
133782	8	406781	5	NULL	NULL	0	NULL	markers 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum concentration of adiponectin and sICAM-1 did not correlate but sICAM-1 was independently , positively associated with sVCAM-1 ( p & lt ; 0.0001 ) and negatively with markers of insulin resistance and inflammation , namely atherogenic index log ( triglycerides/HDL-cholesterol ) ( p & lt ; 0.0001 ) , hs-CRP ( p & lt ; 0.001 ) and HOMA ( p & lt ; 0.05 ) .
	manualset3
133784	9	406781	5	NULL	NULL	0	NULL	insulin resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum concentration of adiponectin and sICAM-1 did not correlate but sICAM-1 was independently , positively associated with sVCAM-1 ( p & lt ; 0.0001 ) and negatively with markers of insulin resistance and inflammation , namely atherogenic index log ( triglycerides/HDL-cholesterol ) ( p & lt ; 0.0001 ) , hs-CRP ( p & lt ; 0.001 ) and HOMA ( p & lt ; 0.05 ) .
	manualset3
133786	10	406781	5	NULL	NULL	0	NULL	inflammation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum concentration of adiponectin and sICAM-1 did not correlate but sICAM-1 was independently , positively associated with sVCAM-1 ( p & lt ; 0.0001 ) and negatively with markers of insulin resistance and inflammation , namely atherogenic index log ( triglycerides/HDL-cholesterol ) ( p & lt ; 0.0001 ) , hs-CRP ( p & lt ; 0.001 ) and HOMA ( p & lt ; 0.05 ) .
	manualset3
133787	11	406781	5	NULL	NULL	0	NULL	atherogenic index log ( triglycerides/HDL-cholesterol )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum concentration of adiponectin and sICAM-1 did not correlate but sICAM-1 was independently , positively associated with sVCAM-1 ( p & lt ; 0.0001 ) and negatively with markers of insulin resistance and inflammation , namely atherogenic index log ( triglycerides/HDL-cholesterol ) ( p & lt ; 0.0001 ) , hs-CRP ( p & lt ; 0.001 ) and HOMA ( p & lt ; 0.05 ) .
	manualset3
133788	12	406781	5	NULL	NULL	0	NULL	p & lt ; 0.0001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum concentration of adiponectin and sICAM-1 did not correlate but sICAM-1 was independently , positively associated with sVCAM-1 ( p & lt ; 0.0001 ) and negatively with markers of insulin resistance and inflammation , namely atherogenic index log ( triglycerides/HDL-cholesterol ) ( p & lt ; 0.0001 ) , hs-CRP ( p & lt ; 0.001 ) and HOMA ( p & lt ; 0.05 ) .
	manualset3
133789	13	406781	5	NULL	NULL	0	NULL	hs-CRP 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum concentration of adiponectin and sICAM-1 did not correlate but sICAM-1 was independently , positively associated with sVCAM-1 ( p & lt ; 0.0001 ) and negatively with markers of insulin resistance and inflammation , namely atherogenic index log ( triglycerides/HDL-cholesterol ) ( p & lt ; 0.0001 ) , hs-CRP ( p & lt ; 0.001 ) and HOMA ( p & lt ; 0.05 ) .
	manualset3
133790	14	406781	5	NULL	NULL	0	NULL	p & lt ; 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum concentration of adiponectin and sICAM-1 did not correlate but sICAM-1 was independently , positively associated with sVCAM-1 ( p & lt ; 0.0001 ) and negatively with markers of insulin resistance and inflammation , namely atherogenic index log ( triglycerides/HDL-cholesterol ) ( p & lt ; 0.0001 ) , hs-CRP ( p & lt ; 0.001 ) and HOMA ( p & lt ; 0.05 ) .
	manualset3
133791	15	406781	5	NULL	NULL	0	NULL	HOMA 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum concentration of adiponectin and sICAM-1 did not correlate but sICAM-1 was independently , positively associated with sVCAM-1 ( p & lt ; 0.0001 ) and negatively with markers of insulin resistance and inflammation , namely atherogenic index log ( triglycerides/HDL-cholesterol ) ( p & lt ; 0.0001 ) , hs-CRP ( p & lt ; 0.001 ) and HOMA ( p & lt ; 0.05 ) .
	manualset3
133792	16	406781	5	NULL	NULL	0	NULL	p & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum concentration of adiponectin and sICAM-1 did not correlate but sICAM-1 was independently , positively associated with sVCAM-1 ( p & lt ; 0.0001 ) and negatively with markers of insulin resistance and inflammation , namely atherogenic index log ( triglycerides/HDL-cholesterol ) ( p & lt ; 0.0001 ) , hs-CRP ( p & lt ; 0.001 ) and HOMA ( p & lt ; 0.05 ) .
	manualset3
133793	1	406782	5	NULL	NULL	0	NULL	Serum concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum concentrations of progesterone at the time of necropsy were 0.47 + / - 0.02 , 0.18 + / - 0.02 and 0.10 + / - 0.01 mumol/l respectively .
	manualset3
133794	2	406782	5	NULL	NULL	0	NULL	progesterone 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum concentrations of progesterone at the time of necropsy were 0.47 + / - 0.02 , 0.18 + / - 0.02 and 0.10 + / - 0.01 mumol/l respectively .
	manualset3
133795	3	406782	5	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum concentrations of progesterone at the time of necropsy were 0.47 + / - 0.02 , 0.18 + / - 0.02 and 0.10 + / - 0.01 mumol/l respectively .
	manualset3
133796	4	406782	5	NULL	NULL	0	NULL	necropsy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum concentrations of progesterone at the time of necropsy were 0.47 + / - 0.02 , 0.18 + / - 0.02 and 0.10 + / - 0.01 mumol/l respectively .
	manualset3
133797	5	406782	5	NULL	NULL	NULL	NULL	0.47 + / - 0.02 mumol/l	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Serum concentrations of progesterone at the time of necropsy were 0.47 + / - 0.02 , 0.18 + / - 0.02 and 0.10 + / - 0.01 mumol/l respectively .
	manualset3
133798	6	406782	5	NULL	NULL	NULL	NULL	0.18 + / - 0.02 mumol/l	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Serum concentrations of progesterone at the time of necropsy were 0.47 + / - 0.02 , 0.18 + / - 0.02 and 0.10 + / - 0.01 mumol/l respectively .
	manualset3
133799	7	406782	5	NULL	NULL	0	NULL	0.10 + / - 0.01 mumol/l 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum concentrations of progesterone at the time of necropsy were 0.47 + / - 0.02 , 0.18 + / - 0.02 and 0.10 + / - 0.01 mumol/l respectively .
	manualset3
133800	1	406783	5	NULL	NULL	0	NULL	Serum cortisol values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum cortisol values , superior vena cava flow and illness severity scores in very low birth weight infants .
	manualset3
133801	2	406783	5	NULL	NULL	0	NULL	superior vena cava flow	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum cortisol values , superior vena cava flow and illness severity scores in very low birth weight infants .
	manualset3
133802	3	406783	5	NULL	NULL	0	NULL	illness severity scores	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum cortisol values , superior vena cava flow and illness severity scores in very low birth weight infants .
	manualset3
133803	4	406783	5	NULL	NULL	0	NULL	very low birth weight infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum cortisol values , superior vena cava flow and illness severity scores in very low birth weight infants .
	manualset3
133804	1	406784	5	NULL	NULL	0	NULL	Serum creatine phosphokinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum creatine phosphokinase : a probable marker of severity in organophosphorus poisoning .
	manualset3
133805	2	406784	5	NULL	NULL	0	NULL	marker 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum creatine phosphokinase : a probable marker of severity in organophosphorus poisoning .
	manualset3
133806	3	406784	5	NULL	NULL	0	NULL	severity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum creatine phosphokinase : a probable marker of severity in organophosphorus poisoning .
	manualset3
133807	4	406784	5	NULL	NULL	0	NULL	organophosphorus poisoning	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum creatine phosphokinase : a probable marker of severity in organophosphorus poisoning .
	manualset3
133808	1	406785	5	NULL	NULL	0	NULL	Serum enzyme levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum enzyme levels in diagnosis of postoperative myocardial infarction .
	manualset3
133809	2	406785	5	NULL	NULL	0	NULL	diagnosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum enzyme levels in diagnosis of postoperative myocardial infarction .
	manualset3
133810	3	406785	5	NULL	NULL	0	NULL	postoperative myocardial infarction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum enzyme levels in diagnosis of postoperative myocardial infarction .
	manualset3
133811	1	406786	5	NULL	NULL	0	NULL	Serum ferritin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum ferritin in young men during prolonged heavy physical exercise .
	manualset3
133812	2	406786	5	NULL	NULL	0	NULL	young men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum ferritin in young men during prolonged heavy physical exercise .
	manualset3
133813	3	406786	5	NULL	NULL	0	NULL	heavy physical exercise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum ferritin in young men during prolonged heavy physical exercise .
	manualset3
133814	1	406787	5	NULL	NULL	NULL	NULL	Serum immunoglobulin levels	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Serum immunoglobulin ( IgG , IgA , IgM ) and complement ( C3 , C4 ) levels were within normal limits in both patient groups .
	manualset3
133815	2	406787	5	NULL	NULL	0	NULL	IgG 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum immunoglobulin ( IgG , IgA , IgM ) and complement ( C3 , C4 ) levels were within normal limits in both patient groups .
	manualset3
133816	3	406787	5	NULL	NULL	0	NULL	IgA 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum immunoglobulin ( IgG , IgA , IgM ) and complement ( C3 , C4 ) levels were within normal limits in both patient groups .
	manualset3
133817	4	406787	5	NULL	NULL	0	NULL	IgM 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum immunoglobulin ( IgG , IgA , IgM ) and complement ( C3 , C4 ) levels were within normal limits in both patient groups .
	manualset3
133818	5	406787	5	NULL	NULL	NULL	NULL	complement levels	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Serum immunoglobulin ( IgG , IgA , IgM ) and complement ( C3 , C4 ) levels were within normal limits in both patient groups .
	manualset3
133819	6	406787	5	NULL	NULL	0	NULL	 C3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum immunoglobulin ( IgG , IgA , IgM ) and complement ( C3 , C4 ) levels were within normal limits in both patient groups .
	manualset3
133820	7	406787	5	NULL	NULL	0	NULL	C4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum immunoglobulin ( IgG , IgA , IgM ) and complement ( C3 , C4 ) levels were within normal limits in both patient groups .
	manualset3
133821	8	406787	5	NULL	NULL	0	NULL	normal limits	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum immunoglobulin ( IgG , IgA , IgM ) and complement ( C3 , C4 ) levels were within normal limits in both patient groups .
	manualset3
133822	9	406787	5	NULL	NULL	0	NULL	patient groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum immunoglobulin ( IgG , IgA , IgM ) and complement ( C3 , C4 ) levels were within normal limits in both patient groups .
	manualset3
133823	1	406788	5	NULL	NULL	0	NULL	Serum levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum levels of RIST , RAST , and cortisol of patients with allergic rhinitis .
	manualset3
133824	2	406788	5	NULL	NULL	0	NULL	RIST 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum levels of RIST , RAST , and cortisol of patients with allergic rhinitis .
	manualset3
133825	3	406788	5	NULL	NULL	0	NULL	RAST 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum levels of RIST , RAST , and cortisol of patients with allergic rhinitis .
	manualset3
133826	4	406788	5	NULL	NULL	0	NULL	cortisol 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum levels of RIST , RAST , and cortisol of patients with allergic rhinitis .
	manualset3
133827	5	406788	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum levels of RIST , RAST , and cortisol of patients with allergic rhinitis .
	manualset3
133828	6	406788	5	NULL	NULL	0	NULL	allergic rhinitis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum levels of RIST , RAST , and cortisol of patients with allergic rhinitis .
	manualset3
133829	1	406789	5	NULL	NULL	0	NULL	Serum matrix-metalloproteinase-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum matrix-metalloproteinase-1 is a bona fide prognostic marker for colorectal cancer .
	manualset3
133830	2	406789	5	NULL	NULL	0	NULL	bona fide prognostic marker	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum matrix-metalloproteinase-1 is a bona fide prognostic marker for colorectal cancer .
	manualset3
133831	3	406789	5	NULL	NULL	0	NULL	colorectal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum matrix-metalloproteinase-1 is a bona fide prognostic marker for colorectal cancer .
	manualset3
133832	1	406790	5	NULL	NULL	0	NULL	Serum nm23-HI levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum nm23-HI levels were significantly higher in patients with all of the hematological neoplasms tested ( AML , chronic myelogenous leukemia , acute lymphoblastic leukemia , ( ALL ) myelodysplastic syndrome ( MDS ) and malignant lymphomas ) than in normal controls .
	manualset3
133833	2	406790	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum nm23-HI levels were significantly higher in patients with all of the hematological neoplasms tested ( AML , chronic myelogenous leukemia , acute lymphoblastic leukemia , ( ALL ) myelodysplastic syndrome ( MDS ) and malignant lymphomas ) than in normal controls .
	manualset3
133834	3	406790	5	NULL	NULL	0	NULL	hematological neoplasms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum nm23-HI levels were significantly higher in patients with all of the hematological neoplasms tested ( AML , chronic myelogenous leukemia , acute lymphoblastic leukemia , ( ALL ) myelodysplastic syndrome ( MDS ) and malignant lymphomas ) than in normal controls .
	manualset3
133835	4	406790	5	NULL	NULL	0	NULL	AML	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum nm23-HI levels were significantly higher in patients with all of the hematological neoplasms tested ( AML , chronic myelogenous leukemia , acute lymphoblastic leukemia , ( ALL ) myelodysplastic syndrome ( MDS ) and malignant lymphomas ) than in normal controls .
	manualset3
133836	5	406790	5	NULL	NULL	0	NULL	chronic myelogenous leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum nm23-HI levels were significantly higher in patients with all of the hematological neoplasms tested ( AML , chronic myelogenous leukemia , acute lymphoblastic leukemia , ( ALL ) myelodysplastic syndrome ( MDS ) and malignant lymphomas ) than in normal controls .
	manualset3
133837	6	406790	5	NULL	NULL	0	NULL	acute lymphoblastic leukemia , ( ALL ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum nm23-HI levels were significantly higher in patients with all of the hematological neoplasms tested ( AML , chronic myelogenous leukemia , acute lymphoblastic leukemia , ( ALL ) myelodysplastic syndrome ( MDS ) and malignant lymphomas ) than in normal controls .
	manualset3
133838	7	406790	5	NULL	NULL	0	NULL	myelodysplastic syndrome ( MDS ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum nm23-HI levels were significantly higher in patients with all of the hematological neoplasms tested ( AML , chronic myelogenous leukemia , acute lymphoblastic leukemia , ( ALL ) myelodysplastic syndrome ( MDS ) and malignant lymphomas ) than in normal controls .
	manualset3
133839	8	406790	5	NULL	NULL	0	NULL	malignant lymphomas 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum nm23-HI levels were significantly higher in patients with all of the hematological neoplasms tested ( AML , chronic myelogenous leukemia , acute lymphoblastic leukemia , ( ALL ) myelodysplastic syndrome ( MDS ) and malignant lymphomas ) than in normal controls .
	manualset3
133840	9	406790	5	NULL	NULL	0	NULL	normal controls	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum nm23-HI levels were significantly higher in patients with all of the hematological neoplasms tested ( AML , chronic myelogenous leukemia , acute lymphoblastic leukemia , ( ALL ) myelodysplastic syndrome ( MDS ) and malignant lymphomas ) than in normal controls .
	manualset3
133841	1	406791	5	NULL	NULL	0	NULL	Serum potassium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum potassium increased to higher levels at exhaustion and muscle potassium decreased to lower levels with NAD than with AT or PLAC .
	manualset3
133842	2	406791	5	NULL	NULL	0	NULL	 higher levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum potassium increased to higher levels at exhaustion and muscle potassium decreased to lower levels with NAD than with AT or PLAC .
	manualset3
133843	3	406791	5	NULL	NULL	0	NULL	exhaustion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum potassium increased to higher levels at exhaustion and muscle potassium decreased to lower levels with NAD than with AT or PLAC .
	manualset3
133844	4	406791	5	NULL	NULL	0	NULL	muscle potassium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum potassium increased to higher levels at exhaustion and muscle potassium decreased to lower levels with NAD than with AT or PLAC .
	manualset3
133845	5	406791	5	NULL	NULL	0	NULL	lower levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum potassium increased to higher levels at exhaustion and muscle potassium decreased to lower levels with NAD than with AT or PLAC .
	manualset3
133846	6	406791	5	NULL	NULL	0	NULL	NAD 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum potassium increased to higher levels at exhaustion and muscle potassium decreased to lower levels with NAD than with AT or PLAC .
	manualset3
133847	7	406791	5	NULL	NULL	NULL	NULL	AT 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Serum potassium increased to higher levels at exhaustion and muscle potassium decreased to lower levels with NAD than with AT or PLAC .
	manualset3
133848	8	406791	5	NULL	NULL	0	NULL	PLAC 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum potassium increased to higher levels at exhaustion and muscle potassium decreased to lower levels with NAD than with AT or PLAC .
	manualset3
133849	1	406792	5	NULL	NULL	0	NULL	Serum prolactin levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum prolactin levels at 9 : 00 AM were significantly correlated with peak serum prolactin levels in both male and female patients .
	manualset3
133850	2	406792	5	NULL	NULL	0	NULL	9 : 00 AM	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum prolactin levels at 9 : 00 AM were significantly correlated with peak serum prolactin levels in both male and female patients .
	manualset3
133851	3	406792	5	NULL	NULL	0	NULL	peak serum prolactin levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum prolactin levels at 9 : 00 AM were significantly correlated with peak serum prolactin levels in both male and female patients .
	manualset3
133852	4	406792	5	NULL	NULL	0	NULL	male patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum prolactin levels at 9 : 00 AM were significantly correlated with peak serum prolactin levels in both male and female patients .
	manualset3
133853	5	406792	5	NULL	NULL	0	NULL	female patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum prolactin levels at 9 : 00 AM were significantly correlated with peak serum prolactin levels in both male and female patients .
	manualset3
133854	1	406793	5	NULL	NULL	0	NULL	non-papillary and broad-based tumor 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A non-papillary and broad-based tumor was located in the trigone and bladder neck on cystoscopic examination .
	manualset3
133855	2	406793	5	NULL	NULL	0	NULL	trigone 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A non-papillary and broad-based tumor was located in the trigone and bladder neck on cystoscopic examination .
	manualset3
133856	3	406793	5	NULL	NULL	0	NULL	bladder neck	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A non-papillary and broad-based tumor was located in the trigone and bladder neck on cystoscopic examination .
	manualset3
133857	4	406793	5	NULL	NULL	0	NULL	cystoscopic examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A non-papillary and broad-based tumor was located in the trigone and bladder neck on cystoscopic examination .
	manualset3
133858	1	406794	5	NULL	NULL	0	NULL	Serum prolactin levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum prolactin levels in five patients were extremely high ( above 1 , 200 mIU/l ) .
	manualset3
133859	2	406794	5	NULL	NULL	0	NULL	five 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum prolactin levels in five patients were extremely high ( above 1 , 200 mIU/l ) .
	manualset3
133860	3	406794	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum prolactin levels in five patients were extremely high ( above 1 , 200 mIU/l ) .
	manualset3
133861	4	406794	5	NULL	NULL	0	NULL	1 , 200 mIU/l	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum prolactin levels in five patients were extremely high ( above 1 , 200 mIU/l ) .
	manualset3
133862	1	406795	5	NULL	NULL	0	NULL	Serum protein interference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum protein interference is equivalent to 3.3 plus or minus 1.25 mmol of CO2 per liter and hence is sufficiently constant to be corrected for by use of a serum standard or serum blank .
	manualset3
133863	2	406795	5	NULL	NULL	NULL	NULL	3.3 plus or minus 1.25 mmol CO2 per liter	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Serum protein interference is equivalent to 3.3 plus or minus 1.25 mmol of CO2 per liter and hence is sufficiently constant to be corrected for by use of a serum standard or serum blank .
	manualset3
133865	4	406795	5	NULL	NULL	0	NULL	serum standard	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum protein interference is equivalent to 3.3 plus or minus 1.25 mmol of CO2 per liter and hence is sufficiently constant to be corrected for by use of a serum standard or serum blank .
	manualset3
133866	5	406795	5	NULL	NULL	0	NULL	serum blank	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum protein interference is equivalent to 3.3 plus or minus 1.25 mmol of CO2 per liter and hence is sufficiently constant to be corrected for by use of a serum standard or serum blank .
	manualset3
133867	1	406796	5	NULL	NULL	0	NULL	Serum response factor ( SRF )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum response factor ( SRF ) is a transcription factor that regulates many genes involved in cellular activities such as proliferation , migration , differentiation , angiogenesis , and apoptosis .
	manualset3
133868	2	406796	5	NULL	NULL	0	NULL	transcription factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum response factor ( SRF ) is a transcription factor that regulates many genes involved in cellular activities such as proliferation , migration , differentiation , angiogenesis , and apoptosis .
	manualset3
133869	3	406796	5	NULL	NULL	0	NULL	genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum response factor ( SRF ) is a transcription factor that regulates many genes involved in cellular activities such as proliferation , migration , differentiation , angiogenesis , and apoptosis .
	manualset3
133870	4	406796	5	NULL	NULL	0	NULL	cellular activities 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum response factor ( SRF ) is a transcription factor that regulates many genes involved in cellular activities such as proliferation , migration , differentiation , angiogenesis , and apoptosis .
	manualset3
133871	5	406796	5	NULL	NULL	0	NULL	proliferation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum response factor ( SRF ) is a transcription factor that regulates many genes involved in cellular activities such as proliferation , migration , differentiation , angiogenesis , and apoptosis .
	manualset3
133872	6	406796	5	NULL	NULL	0	NULL	migration 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum response factor ( SRF ) is a transcription factor that regulates many genes involved in cellular activities such as proliferation , migration , differentiation , angiogenesis , and apoptosis .
	manualset3
133873	7	406796	5	NULL	NULL	0	NULL	differentiation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum response factor ( SRF ) is a transcription factor that regulates many genes involved in cellular activities such as proliferation , migration , differentiation , angiogenesis , and apoptosis .
	manualset3
133874	8	406796	5	NULL	NULL	0	NULL	angiogenesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum response factor ( SRF ) is a transcription factor that regulates many genes involved in cellular activities such as proliferation , migration , differentiation , angiogenesis , and apoptosis .
	manualset3
133875	9	406796	5	NULL	NULL	0	NULL	apoptosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum response factor ( SRF ) is a transcription factor that regulates many genes involved in cellular activities such as proliferation , migration , differentiation , angiogenesis , and apoptosis .
	manualset3
133876	1	406797	5	NULL	NULL	0	NULL	Serum retinol level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum retinol , alpha-tocopherol , and beta-carotene levels are not altered by excess ingestion of diacylglycerol-containing plant sterol esters .
	manualset3
133877	2	406797	5	NULL	NULL	0	NULL	serum  alpha-tocopherol  level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum retinol , alpha-tocopherol , and beta-carotene levels are not altered by excess ingestion of diacylglycerol-containing plant sterol esters .
	manualset3
133878	3	406797	5	NULL	NULL	0	NULL	serum beta-carotene level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum retinol , alpha-tocopherol , and beta-carotene levels are not altered by excess ingestion of diacylglycerol-containing plant sterol esters .
	manualset3
133879	4	406797	5	NULL	NULL	0	NULL	ingestion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum retinol , alpha-tocopherol , and beta-carotene levels are not altered by excess ingestion of diacylglycerol-containing plant sterol esters .
	manualset3
133880	5	406797	5	NULL	NULL	0	NULL	diacylglycerol-containing plant sterol esters	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum retinol , alpha-tocopherol , and beta-carotene levels are not altered by excess ingestion of diacylglycerol-containing plant sterol esters .
	manualset3
133881	1	406798	5	NULL	NULL	0	NULL	Serum thyroglobulin levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum thyroglobulin levels equal to or below 20 ng/ml indicate the absence of thyroid carcinoma , and values exceeding 60 ng/ml were indicative of active thyroid cancer but may include some patients without clinical evidence of disease .
	manualset3
133882	2	406798	5	NULL	NULL	0	NULL	20 ng/ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum thyroglobulin levels equal to or below 20 ng/ml indicate the absence of thyroid carcinoma , and values exceeding 60 ng/ml were indicative of active thyroid cancer but may include some patients without clinical evidence of disease .
	manualset3
133883	3	406798	5	NULL	NULL	0	NULL	absence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum thyroglobulin levels equal to or below 20 ng/ml indicate the absence of thyroid carcinoma , and values exceeding 60 ng/ml were indicative of active thyroid cancer but may include some patients without clinical evidence of disease .
	manualset3
133884	4	406798	5	NULL	NULL	0	NULL	thyroid carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum thyroglobulin levels equal to or below 20 ng/ml indicate the absence of thyroid carcinoma , and values exceeding 60 ng/ml were indicative of active thyroid cancer but may include some patients without clinical evidence of disease .
	manualset3
133885	5	406798	5	NULL	NULL	0	NULL	values 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum thyroglobulin levels equal to or below 20 ng/ml indicate the absence of thyroid carcinoma , and values exceeding 60 ng/ml were indicative of active thyroid cancer but may include some patients without clinical evidence of disease .
	manualset3
133886	6	406798	5	NULL	NULL	0	NULL	60 ng/ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum thyroglobulin levels equal to or below 20 ng/ml indicate the absence of thyroid carcinoma , and values exceeding 60 ng/ml were indicative of active thyroid cancer but may include some patients without clinical evidence of disease .
	manualset3
133887	7	406798	5	NULL	NULL	0	NULL	active thyroid cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum thyroglobulin levels equal to or below 20 ng/ml indicate the absence of thyroid carcinoma , and values exceeding 60 ng/ml were indicative of active thyroid cancer but may include some patients without clinical evidence of disease .
	manualset3
133888	8	406798	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum thyroglobulin levels equal to or below 20 ng/ml indicate the absence of thyroid carcinoma , and values exceeding 60 ng/ml were indicative of active thyroid cancer but may include some patients without clinical evidence of disease .
	manualset3
133889	9	406798	5	NULL	NULL	0	NULL	clinical evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum thyroglobulin levels equal to or below 20 ng/ml indicate the absence of thyroid carcinoma , and values exceeding 60 ng/ml were indicative of active thyroid cancer but may include some patients without clinical evidence of disease .
	manualset3
133890	10	406798	5	NULL	NULL	0	NULL	disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum thyroglobulin levels equal to or below 20 ng/ml indicate the absence of thyroid carcinoma , and values exceeding 60 ng/ml were indicative of active thyroid cancer but may include some patients without clinical evidence of disease .
	manualset3
133891	1	406799	5	NULL	NULL	0	NULL	Serum 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum was obtained three hours after intravenous administration of LPS .
	manualset3
133892	2	406799	5	NULL	NULL	0	NULL	three hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum was obtained three hours after intravenous administration of LPS .
	manualset3
133893	3	406799	5	NULL	NULL	0	NULL	intravenous administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum was obtained three hours after intravenous administration of LPS .
	manualset3
133894	4	406799	5	NULL	NULL	0	NULL	LPS 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum was obtained three hours after intravenous administration of LPS .
	manualset3
133895	1	406800	5	NULL	NULL	0	NULL	Seven and 6 of the 14 compounds 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven and 6 of the 14 compounds also blocked the binding of the prototype Norwalk virus ( A and H binder ) to the A and H antigens , respectively .
	manualset3
133896	2	406800	5	NULL	NULL	0	NULL	prototype Norwalk virus ( A and H binder ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven and 6 of the 14 compounds also blocked the binding of the prototype Norwalk virus ( A and H binder ) to the A and H antigens , respectively .
	manualset3
133897	3	406800	5	NULL	NULL	0	NULL	A and H antigens	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven and 6 of the 14 compounds also blocked the binding of the prototype Norwalk virus ( A and H binder ) to the A and H antigens , respectively .
	manualset3
134877	4	406800	5	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven and 6 of the 14 compounds also blocked the binding of the prototype Norwalk virus ( A and H binder ) to the A and H antigens , respectively .
	manualset3
133968	1	406801	5	NULL	NULL	0	NULL	Seven cases	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven cases of an aneurysm of the VA fenestration have been reported .
	manualset3
133969	2	406801	5	NULL	NULL	0	NULL	aneurysm 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven cases of an aneurysm of the VA fenestration have been reported .
	manualset3
133970	3	406801	5	NULL	NULL	0	NULL	 VA fenestration 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven cases of an aneurysm of the VA fenestration have been reported .
	manualset3
133971	1	406802	5	NULL	NULL	0	NULL	Seven extensor tendon relocations	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven extensor tendon relocations were performed .
	manualset3
133972	1	406803	5	NULL	NULL	0	NULL	Seven 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven had complete normalization of blood counts , and four achieved a durable response only after the addition of erythropoietin .
	manualset3
133973	2	406803	5	NULL	NULL	0	NULL	normalization 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven had complete normalization of blood counts , and four achieved a durable response only after the addition of erythropoietin .
	manualset3
133974	3	406803	5	NULL	NULL	0	NULL	blood counts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven had complete normalization of blood counts , and four achieved a durable response only after the addition of erythropoietin .
	manualset3
133975	4	406803	5	NULL	NULL	0	NULL	four 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven had complete normalization of blood counts , and four achieved a durable response only after the addition of erythropoietin .
	manualset3
133976	5	406803	5	NULL	NULL	0	NULL	durable response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven had complete normalization of blood counts , and four achieved a durable response only after the addition of erythropoietin .
	manualset3
133977	6	406803	5	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven had complete normalization of blood counts , and four achieved a durable response only after the addition of erythropoietin .
	manualset3
133978	7	406803	5	NULL	NULL	0	NULL	erythropoietin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven had complete normalization of blood counts , and four achieved a durable response only after the addition of erythropoietin .
	manualset3
133979	1	406804	5	NULL	NULL	0	NULL	Seven 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven mutants of M. xanthus dsp , designated fbd mutants , were isolated from 6 , 983 colonies ; these represent putative fibril receptor-minus mutants .
	manualset3
133980	2	406804	5	NULL	NULL	0	NULL	mutants of M. xanthus dsp 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven mutants of M. xanthus dsp , designated fbd mutants , were isolated from 6 , 983 colonies ; these represent putative fibril receptor-minus mutants .
	manualset3
133981	3	406804	5	NULL	NULL	0	NULL	fbd mutants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven mutants of M. xanthus dsp , designated fbd mutants , were isolated from 6 , 983 colonies ; these represent putative fibril receptor-minus mutants .
	manualset3
133982	4	406804	5	NULL	NULL	0	NULL	 6 , 983 colonies 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven mutants of M. xanthus dsp , designated fbd mutants , were isolated from 6 , 983 colonies ; these represent putative fibril receptor-minus mutants .
	manualset3
133983	5	406804	5	NULL	NULL	0	NULL	putative fibril receptor-minus mutants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven mutants of M. xanthus dsp , designated fbd mutants , were isolated from 6 , 983 colonies ; these represent putative fibril receptor-minus mutants .
	manualset3
133984	1	406805	5	NULL	NULL	0	NULL	Seven 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven of the duodenal ulcer patients with a basal acid output greater than 15.0 meq/hr were Helicobacter pylori-positive , suggesting that the organism can withstand even extreme levels of gastric acidity .
	manualset3
133985	2	406805	5	NULL	NULL	0	NULL	duodenal ulcer patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven of the duodenal ulcer patients with a basal acid output greater than 15.0 meq/hr were Helicobacter pylori-positive , suggesting that the organism can withstand even extreme levels of gastric acidity .
	manualset3
133986	3	406805	5	NULL	NULL	0	NULL	basal acid output 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven of the duodenal ulcer patients with a basal acid output greater than 15.0 meq/hr were Helicobacter pylori-positive , suggesting that the organism can withstand even extreme levels of gastric acidity .
	manualset3
133987	4	406805	5	NULL	NULL	0	NULL	15.0 meq/hr 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven of the duodenal ulcer patients with a basal acid output greater than 15.0 meq/hr were Helicobacter pylori-positive , suggesting that the organism can withstand even extreme levels of gastric acidity .
	manualset3
133988	5	406805	5	NULL	NULL	0	NULL	Helicobacter pylori-positive	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven of the duodenal ulcer patients with a basal acid output greater than 15.0 meq/hr were Helicobacter pylori-positive , suggesting that the organism can withstand even extreme levels of gastric acidity .
	manualset3
133989	6	406805	5	NULL	NULL	0	NULL	organism 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven of the duodenal ulcer patients with a basal acid output greater than 15.0 meq/hr were Helicobacter pylori-positive , suggesting that the organism can withstand even extreme levels of gastric acidity .
	manualset3
133990	7	406805	5	NULL	NULL	0	NULL	extreme levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven of the duodenal ulcer patients with a basal acid output greater than 15.0 meq/hr were Helicobacter pylori-positive , suggesting that the organism can withstand even extreme levels of gastric acidity .
	manualset3
133991	8	406805	5	NULL	NULL	0	NULL	gastric acidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven of the duodenal ulcer patients with a basal acid output greater than 15.0 meq/hr were Helicobacter pylori-positive , suggesting that the organism can withstand even extreme levels of gastric acidity .
	manualset3
133992	1	406806	5	NULL	NULL	0	NULL	Seven 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven of the predicted ORFs were linked to rsaA .
	manualset3
133993	2	406806	5	NULL	NULL	0	NULL	predicted ORFs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven of the predicted ORFs were linked to rsaA .
	manualset3
133994	3	406806	5	NULL	NULL	0	NULL	rsaA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven of the predicted ORFs were linked to rsaA .
	manualset3
133995	1	406807	5	NULL	NULL	0	NULL	Seven patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven patients sustained an acute myocardial infarction ( AMI ) , among whom five underwent a PTCA of an occluded vessel .
	manualset3
133996	2	406807	5	NULL	NULL	0	NULL	acute myocardial infarction ( AMI )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven patients sustained an acute myocardial infarction ( AMI ) , among whom five underwent a PTCA of an occluded vessel .
	manualset3
133997	3	406807	5	NULL	NULL	0	NULL	five 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven patients sustained an acute myocardial infarction ( AMI ) , among whom five underwent a PTCA of an occluded vessel .
	manualset3
133998	4	406807	5	NULL	NULL	0	NULL	PTCA 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven patients sustained an acute myocardial infarction ( AMI ) , among whom five underwent a PTCA of an occluded vessel .
	manualset3
133999	5	406807	5	NULL	NULL	0	NULL	occluded vessel	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven patients sustained an acute myocardial infarction ( AMI ) , among whom five underwent a PTCA of an occluded vessel .
	manualset3
134000	1	406808	5	NULL	NULL	0	NULL	Seven years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven years later , he presented with intermittent aortic insufficiency demonstrated by echocardiography , fluoroscopy and angiography .
	manualset3
134001	2	406808	5	NULL	NULL	0	NULL	intermittent aortic insufficiency 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven years later , he presented with intermittent aortic insufficiency demonstrated by echocardiography , fluoroscopy and angiography .
	manualset3
134002	3	406808	5	NULL	NULL	0	NULL	echocardiography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven years later , he presented with intermittent aortic insufficiency demonstrated by echocardiography , fluoroscopy and angiography .
	manualset3
134003	4	406808	5	NULL	NULL	0	NULL	fluoroscopy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven years later , he presented with intermittent aortic insufficiency demonstrated by echocardiography , fluoroscopy and angiography .
	manualset3
134004	5	406808	5	NULL	NULL	0	NULL	angiography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven years later , he presented with intermittent aortic insufficiency demonstrated by echocardiography , fluoroscopy and angiography .
	manualset3
134005	1	406809	5	NULL	NULL	0	NULL	5 , 5 ' , 6 , 6 ' - tetrachloro-1 , 1 ' , 3 , 3 ' - tetraethyl-imidacarbo-cyanine iodide ( JC-1 )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3 ) Following staining by 5 , 5 ' , 6 , 6 ' - tetrachloro-1 , 1 ' , 3 , 3 ' - tetraethyl-imidacarbo-cyanine iodide ( JC-1 ) , most red-colored mitochondria ( high Deltapsi ) were distributed peripherally around pronuclei and along cell membranes of fresh 2-PN embryos .
	manualset3
134006	2	406809	5	NULL	NULL	0	NULL	red-colored mitochondria ( high Deltapsi )	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3 ) Following staining by 5 , 5 ' , 6 , 6 ' - tetrachloro-1 , 1 ' , 3 , 3 ' - tetraethyl-imidacarbo-cyanine iodide ( JC-1 ) , most red-colored mitochondria ( high Deltapsi ) were distributed peripherally around pronuclei and along cell membranes of fresh 2-PN embryos .
	manualset3
134007	3	406809	5	NULL	NULL	0	NULL	pronuclei 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3 ) Following staining by 5 , 5 ' , 6 , 6 ' - tetrachloro-1 , 1 ' , 3 , 3 ' - tetraethyl-imidacarbo-cyanine iodide ( JC-1 ) , most red-colored mitochondria ( high Deltapsi ) were distributed peripherally around pronuclei and along cell membranes of fresh 2-PN embryos .
	manualset3
134008	4	406809	5	NULL	NULL	0	NULL	cell membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3 ) Following staining by 5 , 5 ' , 6 , 6 ' - tetrachloro-1 , 1 ' , 3 , 3 ' - tetraethyl-imidacarbo-cyanine iodide ( JC-1 ) , most red-colored mitochondria ( high Deltapsi ) were distributed peripherally around pronuclei and along cell membranes of fresh 2-PN embryos .
	manualset3
134009	5	406809	5	NULL	NULL	0	NULL	 fresh 2-PN embryos	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3 ) Following staining by 5 , 5 ' , 6 , 6 ' - tetrachloro-1 , 1 ' , 3 , 3 ' - tetraethyl-imidacarbo-cyanine iodide ( JC-1 ) , most red-colored mitochondria ( high Deltapsi ) were distributed peripherally around pronuclei and along cell membranes of fresh 2-PN embryos .
	manualset3
134010	1	406810	5	NULL	NULL	0	NULL	nonisotopic , immunoelectrophoretic technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A nonisotopic , immunoelectrophoretic technique was used to analyze the characteristics of opioid-evoked activation of Gi2 / G ( x/z ) transducer proteins of mouse periaqueductal gray matter membranes .
	manualset3
134011	2	406810	5	NULL	NULL	0	NULL	characteristics 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A nonisotopic , immunoelectrophoretic technique was used to analyze the characteristics of opioid-evoked activation of Gi2 / G ( x/z ) transducer proteins of mouse periaqueductal gray matter membranes .
	manualset3
134012	3	406810	5	NULL	NULL	0	NULL	opioid-evoked activation of Gi2 / G ( x/z ) transducer proteins 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A nonisotopic , immunoelectrophoretic technique was used to analyze the characteristics of opioid-evoked activation of Gi2 / G ( x/z ) transducer proteins of mouse periaqueductal gray matter membranes .
	manualset3
134878	4	406810	5	NULL	NULL	0	NULL	mouse periaqueductal gray matter membranes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A nonisotopic , immunoelectrophoretic technique was used to analyze the characteristics of opioid-evoked activation of Gi2 / G ( x/z ) transducer proteins of mouse periaqueductal gray matter membranes .
	manualset3
134013	1	406811	5	NULL	NULL	0	NULL	Seventy-two percent 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy-two percent of the PTCA patients underwent coronary stenting with an associated incremental cost of $ 1 , 244 .
	manualset3
134014	2	406811	5	NULL	NULL	0	NULL	PTCA patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy-two percent of the PTCA patients underwent coronary stenting with an associated incremental cost of $ 1 , 244 .
	manualset3
134015	3	406811	5	NULL	NULL	0	NULL	coronary stenting	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy-two percent of the PTCA patients underwent coronary stenting with an associated incremental cost of $ 1 , 244 .
	manualset3
134016	4	406811	5	NULL	NULL	0	NULL	 incremental cost	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy-two percent of the PTCA patients underwent coronary stenting with an associated incremental cost of $ 1 , 244 .
	manualset3
134017	5	406811	5	NULL	NULL	0	NULL	 $ 1 , 244 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy-two percent of the PTCA patients underwent coronary stenting with an associated incremental cost of $ 1 , 244 .
	manualset3
134018	1	406812	5	NULL	NULL	0	NULL	Seventy-two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy-two unipolar QRS-inhibited demand pacemakers were examined by provoking myopotential interference by exercise .
	manualset3
134019	2	406812	5	NULL	NULL	0	NULL	unipolar QRS-inhibited demand pacemakers	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy-two unipolar QRS-inhibited demand pacemakers were examined by provoking myopotential interference by exercise .
	manualset3
134020	3	406812	5	NULL	NULL	0	NULL	provoking myopotential interference 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy-two unipolar QRS-inhibited demand pacemakers were examined by provoking myopotential interference by exercise .
	manualset3
134021	4	406812	5	NULL	NULL	0	NULL	exercise 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy-two unipolar QRS-inhibited demand pacemakers were examined by provoking myopotential interference by exercise .
	manualset3
134022	1	406813	5	NULL	NULL	0	NULL	Seventy 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy social workers were sampled , with equal subsamples representing the five largest fields of practice in social work .
	manualset3
134023	2	406813	5	NULL	NULL	0	NULL	social workers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy social workers were sampled , with equal subsamples representing the five largest fields of practice in social work .
	manualset3
134024	3	406813	5	NULL	NULL	0	NULL	equal subsamples	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy social workers were sampled , with equal subsamples representing the five largest fields of practice in social work .
	manualset3
134025	4	406813	5	NULL	NULL	0	NULL	five 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy social workers were sampled , with equal subsamples representing the five largest fields of practice in social work .
	manualset3
134026	5	406813	5	NULL	NULL	0	NULL	fields of practice	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy social workers were sampled , with equal subsamples representing the five largest fields of practice in social work .
	manualset3
134027	6	406813	5	NULL	NULL	0	NULL	social work	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy social workers were sampled , with equal subsamples representing the five largest fields of practice in social work .
	manualset3
134028	1	406814	5	NULL	NULL	0	NULL	Seventy specimens	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy specimens of normal endometrium ( n = 13 ) and cervix ( n = 12 ) , endometrial hyperplasia ( n = 4 ) , cervical dysplasia ( n = 20 ) , endometrial ( n = 11 ) and cervical carcinoma ( n = 8 ) and uterine metastases of mammary carcinomas ( n = 2 ) have been analyzed for c-erB-2 expression with immunohistochemistry employing a monoclonal anti ERBB-2 antibody and Northern-blot hybridization using single stranded RNA probes .
	manualset3
134029	2	406814	5	NULL	NULL	0	NULL	normal endometrium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy specimens of normal endometrium ( n = 13 ) and cervix ( n = 12 ) , endometrial hyperplasia ( n = 4 ) , cervical dysplasia ( n = 20 ) , endometrial ( n = 11 ) and cervical carcinoma ( n = 8 ) and uterine metastases of mammary carcinomas ( n = 2 ) have been analyzed for c-erB-2 expression with immunohistochemistry employing a monoclonal anti ERBB-2 antibody and Northern-blot hybridization using single stranded RNA probes .
	manualset3
134030	3	406814	5	NULL	NULL	0	NULL	n = 13	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy specimens of normal endometrium ( n = 13 ) and cervix ( n = 12 ) , endometrial hyperplasia ( n = 4 ) , cervical dysplasia ( n = 20 ) , endometrial ( n = 11 ) and cervical carcinoma ( n = 8 ) and uterine metastases of mammary carcinomas ( n = 2 ) have been analyzed for c-erB-2 expression with immunohistochemistry employing a monoclonal anti ERBB-2 antibody and Northern-blot hybridization using single stranded RNA probes .
	manualset3
134031	4	406814	5	NULL	NULL	0	NULL	cervix 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy specimens of normal endometrium ( n = 13 ) and cervix ( n = 12 ) , endometrial hyperplasia ( n = 4 ) , cervical dysplasia ( n = 20 ) , endometrial ( n = 11 ) and cervical carcinoma ( n = 8 ) and uterine metastases of mammary carcinomas ( n = 2 ) have been analyzed for c-erB-2 expression with immunohistochemistry employing a monoclonal anti ERBB-2 antibody and Northern-blot hybridization using single stranded RNA probes .
	manualset3
134032	5	406814	5	NULL	NULL	0	NULL	n = 12	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy specimens of normal endometrium ( n = 13 ) and cervix ( n = 12 ) , endometrial hyperplasia ( n = 4 ) , cervical dysplasia ( n = 20 ) , endometrial ( n = 11 ) and cervical carcinoma ( n = 8 ) and uterine metastases of mammary carcinomas ( n = 2 ) have been analyzed for c-erB-2 expression with immunohistochemistry employing a monoclonal anti ERBB-2 antibody and Northern-blot hybridization using single stranded RNA probes .
	manualset3
134033	6	406814	5	NULL	NULL	0	NULL	endometrial hyperplasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy specimens of normal endometrium ( n = 13 ) and cervix ( n = 12 ) , endometrial hyperplasia ( n = 4 ) , cervical dysplasia ( n = 20 ) , endometrial ( n = 11 ) and cervical carcinoma ( n = 8 ) and uterine metastases of mammary carcinomas ( n = 2 ) have been analyzed for c-erB-2 expression with immunohistochemistry employing a monoclonal anti ERBB-2 antibody and Northern-blot hybridization using single stranded RNA probes .
	manualset3
134034	7	406814	5	NULL	NULL	0	NULL	 n = 4 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy specimens of normal endometrium ( n = 13 ) and cervix ( n = 12 ) , endometrial hyperplasia ( n = 4 ) , cervical dysplasia ( n = 20 ) , endometrial ( n = 11 ) and cervical carcinoma ( n = 8 ) and uterine metastases of mammary carcinomas ( n = 2 ) have been analyzed for c-erB-2 expression with immunohistochemistry employing a monoclonal anti ERBB-2 antibody and Northern-blot hybridization using single stranded RNA probes .
	manualset3
134035	8	406814	5	NULL	NULL	0	NULL	cervical dysplasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy specimens of normal endometrium ( n = 13 ) and cervix ( n = 12 ) , endometrial hyperplasia ( n = 4 ) , cervical dysplasia ( n = 20 ) , endometrial ( n = 11 ) and cervical carcinoma ( n = 8 ) and uterine metastases of mammary carcinomas ( n = 2 ) have been analyzed for c-erB-2 expression with immunohistochemistry employing a monoclonal anti ERBB-2 antibody and Northern-blot hybridization using single stranded RNA probes .
	manualset3
134036	9	406814	5	NULL	NULL	0	NULL	n = 20	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy specimens of normal endometrium ( n = 13 ) and cervix ( n = 12 ) , endometrial hyperplasia ( n = 4 ) , cervical dysplasia ( n = 20 ) , endometrial ( n = 11 ) and cervical carcinoma ( n = 8 ) and uterine metastases of mammary carcinomas ( n = 2 ) have been analyzed for c-erB-2 expression with immunohistochemistry employing a monoclonal anti ERBB-2 antibody and Northern-blot hybridization using single stranded RNA probes .
	manualset3
134037	10	406814	5	NULL	NULL	0	NULL	endometrial carcinoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy specimens of normal endometrium ( n = 13 ) and cervix ( n = 12 ) , endometrial hyperplasia ( n = 4 ) , cervical dysplasia ( n = 20 ) , endometrial ( n = 11 ) and cervical carcinoma ( n = 8 ) and uterine metastases of mammary carcinomas ( n = 2 ) have been analyzed for c-erB-2 expression with immunohistochemistry employing a monoclonal anti ERBB-2 antibody and Northern-blot hybridization using single stranded RNA probes .
	manualset3
134038	11	406814	5	NULL	NULL	0	NULL	n = 11	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy specimens of normal endometrium ( n = 13 ) and cervix ( n = 12 ) , endometrial hyperplasia ( n = 4 ) , cervical dysplasia ( n = 20 ) , endometrial ( n = 11 ) and cervical carcinoma ( n = 8 ) and uterine metastases of mammary carcinomas ( n = 2 ) have been analyzed for c-erB-2 expression with immunohistochemistry employing a monoclonal anti ERBB-2 antibody and Northern-blot hybridization using single stranded RNA probes .
	manualset3
134039	12	406814	5	NULL	NULL	0	NULL	cervical carcinoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy specimens of normal endometrium ( n = 13 ) and cervix ( n = 12 ) , endometrial hyperplasia ( n = 4 ) , cervical dysplasia ( n = 20 ) , endometrial ( n = 11 ) and cervical carcinoma ( n = 8 ) and uterine metastases of mammary carcinomas ( n = 2 ) have been analyzed for c-erB-2 expression with immunohistochemistry employing a monoclonal anti ERBB-2 antibody and Northern-blot hybridization using single stranded RNA probes .
	manualset3
134040	13	406814	5	NULL	NULL	0	NULL	 n = 8	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy specimens of normal endometrium ( n = 13 ) and cervix ( n = 12 ) , endometrial hyperplasia ( n = 4 ) , cervical dysplasia ( n = 20 ) , endometrial ( n = 11 ) and cervical carcinoma ( n = 8 ) and uterine metastases of mammary carcinomas ( n = 2 ) have been analyzed for c-erB-2 expression with immunohistochemistry employing a monoclonal anti ERBB-2 antibody and Northern-blot hybridization using single stranded RNA probes .
	manualset3
134306	14	406814	5	NULL	NULL	0	NULL	uterine metastases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy specimens of normal endometrium ( n = 13 ) and cervix ( n = 12 ) , endometrial hyperplasia ( n = 4 ) , cervical dysplasia ( n = 20 ) , endometrial ( n = 11 ) and cervical carcinoma ( n = 8 ) and uterine metastases of mammary carcinomas ( n = 2 ) have been analyzed for c-erB-2 expression with immunohistochemistry employing a monoclonal anti ERBB-2 antibody and Northern-blot hybridization using single stranded RNA probes .
	manualset3
134307	15	406814	5	NULL	NULL	0	NULL	mammary carcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy specimens of normal endometrium ( n = 13 ) and cervix ( n = 12 ) , endometrial hyperplasia ( n = 4 ) , cervical dysplasia ( n = 20 ) , endometrial ( n = 11 ) and cervical carcinoma ( n = 8 ) and uterine metastases of mammary carcinomas ( n = 2 ) have been analyzed for c-erB-2 expression with immunohistochemistry employing a monoclonal anti ERBB-2 antibody and Northern-blot hybridization using single stranded RNA probes .
	manualset3
134308	16	406814	5	NULL	NULL	0	NULL	 n = 2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy specimens of normal endometrium ( n = 13 ) and cervix ( n = 12 ) , endometrial hyperplasia ( n = 4 ) , cervical dysplasia ( n = 20 ) , endometrial ( n = 11 ) and cervical carcinoma ( n = 8 ) and uterine metastases of mammary carcinomas ( n = 2 ) have been analyzed for c-erB-2 expression with immunohistochemistry employing a monoclonal anti ERBB-2 antibody and Northern-blot hybridization using single stranded RNA probes .
	manualset3
134309	17	406814	5	NULL	NULL	0	NULL	c-erB-2 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy specimens of normal endometrium ( n = 13 ) and cervix ( n = 12 ) , endometrial hyperplasia ( n = 4 ) , cervical dysplasia ( n = 20 ) , endometrial ( n = 11 ) and cervical carcinoma ( n = 8 ) and uterine metastases of mammary carcinomas ( n = 2 ) have been analyzed for c-erB-2 expression with immunohistochemistry employing a monoclonal anti ERBB-2 antibody and Northern-blot hybridization using single stranded RNA probes .
	manualset3
134310	18	406814	5	NULL	NULL	0	NULL	immunohistochemistry 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy specimens of normal endometrium ( n = 13 ) and cervix ( n = 12 ) , endometrial hyperplasia ( n = 4 ) , cervical dysplasia ( n = 20 ) , endometrial ( n = 11 ) and cervical carcinoma ( n = 8 ) and uterine metastases of mammary carcinomas ( n = 2 ) have been analyzed for c-erB-2 expression with immunohistochemistry employing a monoclonal anti ERBB-2 antibody and Northern-blot hybridization using single stranded RNA probes .
	manualset3
134311	19	406814	5	NULL	NULL	0	NULL	monoclonal anti ERBB-2 antibody 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy specimens of normal endometrium ( n = 13 ) and cervix ( n = 12 ) , endometrial hyperplasia ( n = 4 ) , cervical dysplasia ( n = 20 ) , endometrial ( n = 11 ) and cervical carcinoma ( n = 8 ) and uterine metastases of mammary carcinomas ( n = 2 ) have been analyzed for c-erB-2 expression with immunohistochemistry employing a monoclonal anti ERBB-2 antibody and Northern-blot hybridization using single stranded RNA probes .
	manualset3
134312	20	406814	5	NULL	NULL	0	NULL	Northern-blot hybridization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy specimens of normal endometrium ( n = 13 ) and cervix ( n = 12 ) , endometrial hyperplasia ( n = 4 ) , cervical dysplasia ( n = 20 ) , endometrial ( n = 11 ) and cervical carcinoma ( n = 8 ) and uterine metastases of mammary carcinomas ( n = 2 ) have been analyzed for c-erB-2 expression with immunohistochemistry employing a monoclonal anti ERBB-2 antibody and Northern-blot hybridization using single stranded RNA probes .
	manualset3
134313	21	406814	5	NULL	NULL	0	NULL	single stranded RNA probes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventy specimens of normal endometrium ( n = 13 ) and cervix ( n = 12 ) , endometrial hyperplasia ( n = 4 ) , cervical dysplasia ( n = 20 ) , endometrial ( n = 11 ) and cervical carcinoma ( n = 8 ) and uterine metastases of mammary carcinomas ( n = 2 ) have been analyzed for c-erB-2 expression with immunohistochemistry employing a monoclonal anti ERBB-2 antibody and Northern-blot hybridization using single stranded RNA probes .
	manualset3
134314	1	406815	5	NULL	NULL	0	NULL	mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several , otherwise rare mutations have been detected , such as : I148T , Q552X , 457TAT -- ) G , R1006H , 2907delTT , 3667ins4 , A559T and G576A .
	manualset3
134318	2	406815	5	NULL	NULL	0	NULL	I148T	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Several , otherwise rare mutations have been detected , such as : I148T , Q552X , 457TAT -- ) G , R1006H , 2907delTT , 3667ins4 , A559T and G576A .
	manualset3
134319	3	406815	5	NULL	NULL	0	NULL	Q552X	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Several , otherwise rare mutations have been detected , such as : I148T , Q552X , 457TAT -- ) G , R1006H , 2907delTT , 3667ins4 , A559T and G576A .
	manualset3
134320	4	406815	5	NULL	NULL	0	NULL	457TAT -- ) G 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Several , otherwise rare mutations have been detected , such as : I148T , Q552X , 457TAT -- ) G , R1006H , 2907delTT , 3667ins4 , A559T and G576A .
	manualset3
134321	5	406815	5	NULL	NULL	0	NULL	R1006H 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Several , otherwise rare mutations have been detected , such as : I148T , Q552X , 457TAT -- ) G , R1006H , 2907delTT , 3667ins4 , A559T and G576A .
	manualset3
134322	6	406815	5	NULL	NULL	0	NULL	2907delTT 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Several , otherwise rare mutations have been detected , such as : I148T , Q552X , 457TAT -- ) G , R1006H , 2907delTT , 3667ins4 , A559T and G576A .
	manualset3
134323	7	406815	5	NULL	NULL	0	NULL	3667ins4 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Several , otherwise rare mutations have been detected , such as : I148T , Q552X , 457TAT -- ) G , R1006H , 2907delTT , 3667ins4 , A559T and G576A .
	manualset3
134324	8	406815	5	NULL	NULL	0	NULL	A559T 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Several , otherwise rare mutations have been detected , such as : I148T , Q552X , 457TAT -- ) G , R1006H , 2907delTT , 3667ins4 , A559T and G576A .
	manualset3
134325	9	406815	5	NULL	NULL	0	NULL	G576A 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Several , otherwise rare mutations have been detected , such as : I148T , Q552X , 457TAT -- ) G , R1006H , 2907delTT , 3667ins4 , A559T and G576A .
	manualset3
134326	1	406816	5	NULL	NULL	0	NULL	nonsurgical treatment regimen	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A nonsurgical treatment regimen for metatarsus adductus utilizing orthoses .
	manualset3
134328	2	406816	5	NULL	NULL	0	NULL	metatarsus adductus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A nonsurgical treatment regimen for metatarsus adductus utilizing orthoses .
	manualset3
134331	3	406816	5	NULL	NULL	0	NULL	orthoses 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	A nonsurgical treatment regimen for metatarsus adductus utilizing orthoses .
	manualset3
134334	1	406817	5	NULL	NULL	0	NULL	BRCA1 mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several BRCA1 mutations have now been found to occur in geographically diverse breast and ovarian cancer families .
	manualset3
134335	2	406817	5	NULL	NULL	0	NULL	breast cancer families	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Several BRCA1 mutations have now been found to occur in geographically diverse breast and ovarian cancer families .
	manualset3
134336	3	406817	5	NULL	NULL	0	NULL	ovarian cancer families	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Several BRCA1 mutations have now been found to occur in geographically diverse breast and ovarian cancer families .
	manualset3
134337	1	406818	5	NULL	NULL	0	NULL	VEP parameters	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several VEP parameters were found changing in dependence of the arousal level : the VEP latency , the amplitude of the second negative component ( N41 ) , and the voltage of the positive component between 60 and 80 ms after the light flash .
	manualset3
134338	2	406818	5	NULL	NULL	0	NULL	dependence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Several VEP parameters were found changing in dependence of the arousal level : the VEP latency , the amplitude of the second negative component ( N41 ) , and the voltage of the positive component between 60 and 80 ms after the light flash .
	manualset3
134339	3	406818	5	NULL	NULL	0	NULL	arousal level	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several VEP parameters were found changing in dependence of the arousal level : the VEP latency , the amplitude of the second negative component ( N41 ) , and the voltage of the positive component between 60 and 80 ms after the light flash .
	manualset3
134340	4	406818	5	NULL	NULL	0	NULL	VEP latency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several VEP parameters were found changing in dependence of the arousal level : the VEP latency , the amplitude of the second negative component ( N41 ) , and the voltage of the positive component between 60 and 80 ms after the light flash .
	manualset3
134341	5	406818	5	NULL	NULL	0	NULL	amplitude 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several VEP parameters were found changing in dependence of the arousal level : the VEP latency , the amplitude of the second negative component ( N41 ) , and the voltage of the positive component between 60 and 80 ms after the light flash .
	manualset3
134342	6	406818	5	NULL	NULL	0	NULL	second negative component ( N41 )	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several VEP parameters were found changing in dependence of the arousal level : the VEP latency , the amplitude of the second negative component ( N41 ) , and the voltage of the positive component between 60 and 80 ms after the light flash .
	manualset3
134343	7	406818	5	NULL	NULL	0	NULL	voltage 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several VEP parameters were found changing in dependence of the arousal level : the VEP latency , the amplitude of the second negative component ( N41 ) , and the voltage of the positive component between 60 and 80 ms after the light flash .
	manualset3
134344	8	406818	5	NULL	NULL	0	NULL	positive component	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several VEP parameters were found changing in dependence of the arousal level : the VEP latency , the amplitude of the second negative component ( N41 ) , and the voltage of the positive component between 60 and 80 ms after the light flash .
	manualset3
134345	9	406818	5	NULL	NULL	0	NULL	60ms	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Several VEP parameters were found changing in dependence of the arousal level : the VEP latency , the amplitude of the second negative component ( N41 ) , and the voltage of the positive component between 60 and 80 ms after the light flash .
	manualset3
134346	10	406818	5	NULL	NULL	0	NULL	80ms	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Several VEP parameters were found changing in dependence of the arousal level : the VEP latency , the amplitude of the second negative component ( N41 ) , and the voltage of the positive component between 60 and 80 ms after the light flash .
	manualset3
134347	11	406818	5	NULL	NULL	0	NULL	light flash	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Several VEP parameters were found changing in dependence of the arousal level : the VEP latency , the amplitude of the second negative component ( N41 ) , and the voltage of the positive component between 60 and 80 ms after the light flash .
	manualset3
134348	1	406819	5	NULL	NULL	0	NULL	aryl pyridyl carbinols	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Several aryl pyridyl carbinols were obtained in high yields .
	manualset3
134349	2	406819	5	NULL	NULL	0	NULL	high yields	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several aryl pyridyl carbinols were obtained in high yields .
	manualset3
134350	1	406820	5	NULL	NULL	0	NULL	cDNA clones 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Several cDNA clones of the La antigen recognized by certain lupus autoantibodies were isolated from lambda gt11 expression libraries made from human liver .
	manualset3
134351	2	406820	5	NULL	NULL	0	NULL	La antigen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Several cDNA clones of the La antigen recognized by certain lupus autoantibodies were isolated from lambda gt11 expression libraries made from human liver .
	manualset3
134352	3	406820	5	NULL	NULL	0	NULL	lupus autoantibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Several cDNA clones of the La antigen recognized by certain lupus autoantibodies were isolated from lambda gt11 expression libraries made from human liver .
	manualset3
134353	4	406820	5	NULL	NULL	0	NULL	lambda gt11 expression libraries	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Several cDNA clones of the La antigen recognized by certain lupus autoantibodies were isolated from lambda gt11 expression libraries made from human liver .
	manualset3
134354	5	406820	5	NULL	NULL	0	NULL	human liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Several cDNA clones of the La antigen recognized by certain lupus autoantibodies were isolated from lambda gt11 expression libraries made from human liver .
	manualset3
134355	1	406821	5	NULL	NULL	0	NULL	clinical finding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Several clinical and experimental findings point towards IL-2 as a crucial mediator inducing immunologic reaction against human follicle in alopecia areata .
	manualset3
134356	2	406821	5	NULL	NULL	0	NULL	experimental finding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Several clinical and experimental findings point towards IL-2 as a crucial mediator inducing immunologic reaction against human follicle in alopecia areata .
	manualset3
134357	3	406821	5	NULL	NULL	0	NULL	 IL-2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Several clinical and experimental findings point towards IL-2 as a crucial mediator inducing immunologic reaction against human follicle in alopecia areata .
	manualset3
134358	4	406821	5	NULL	NULL	0	NULL	crucial mediator 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Several clinical and experimental findings point towards IL-2 as a crucial mediator inducing immunologic reaction against human follicle in alopecia areata .
	manualset3
134359	5	406821	5	NULL	NULL	0	NULL	immunologic reaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several clinical and experimental findings point towards IL-2 as a crucial mediator inducing immunologic reaction against human follicle in alopecia areata .
	manualset3
134360	6	406821	5	NULL	NULL	0	NULL	human follicle 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Several clinical and experimental findings point towards IL-2 as a crucial mediator inducing immunologic reaction against human follicle in alopecia areata .
	manualset3
134361	7	406821	5	NULL	NULL	0	NULL	alopecia areata 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Several clinical and experimental findings point towards IL-2 as a crucial mediator inducing immunologic reaction against human follicle in alopecia areata .
	manualset3
134362	1	406822	5	NULL	NULL	0	NULL	clonal cell lines 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Several clonal cell lines derived from TCL-Fuj and 2M cells had characteristics similar to the respective parent cell lines .
	manualset3
134363	2	406822	5	NULL	NULL	0	NULL	TCL-Fuj cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Several clonal cell lines derived from TCL-Fuj and 2M cells had characteristics similar to the respective parent cell lines .
	manualset3
134364	3	406822	5	NULL	NULL	0	NULL	 2M cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Several clonal cell lines derived from TCL-Fuj and 2M cells had characteristics similar to the respective parent cell lines .
	manualset3
134365	4	406822	5	NULL	NULL	0	NULL	parent cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Several clonal cell lines derived from TCL-Fuj and 2M cells had characteristics similar to the respective parent cell lines .
	manualset3
134366	1	406823	5	NULL	NULL	0	NULL	conditions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Several conditions of pregnancy have similar presentations to the initial , often nonspecific manifestations of RMSF .
	manualset3
134367	2	406823	5	NULL	NULL	0	NULL	pregnancy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Several conditions of pregnancy have similar presentations to the initial , often nonspecific manifestations of RMSF .
	manualset3
134368	3	406823	5	NULL	NULL	0	NULL	presentations 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Several conditions of pregnancy have similar presentations to the initial , often nonspecific manifestations of RMSF .
	manualset3
134369	4	406823	5	NULL	NULL	0	NULL	nonspecific manifestations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Several conditions of pregnancy have similar presentations to the initial , often nonspecific manifestations of RMSF .
	manualset3
134370	5	406823	5	NULL	NULL	0	NULL	RMSF 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Several conditions of pregnancy have similar presentations to the initial , often nonspecific manifestations of RMSF .
	manualset3
134371	1	406824	5	NULL	NULL	0	NULL	female karyotype ( 60 , XX )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A normal female karyotype ( 60 , XX ) was detected in metaphase spreads obtained from cultured peripheral lymphocytes .
	manualset3
134372	2	406824	5	NULL	NULL	0	NULL	metaphase spreads	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A normal female karyotype ( 60 , XX ) was detected in metaphase spreads obtained from cultured peripheral lymphocytes .
	manualset3
134373	3	406824	5	NULL	NULL	0	NULL	cultured peripheral lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A normal female karyotype ( 60 , XX ) was detected in metaphase spreads obtained from cultured peripheral lymphocytes .
	manualset3
134374	1	406825	5	NULL	NULL	0	NULL	cyclic memory attractors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several cyclic memory attractors that correspond to several simple motions of the object in two-dimensional space are embedded .
	manualset3
134375	2	406825	5	NULL	NULL	0	NULL	simple motions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Several cyclic memory attractors that correspond to several simple motions of the object in two-dimensional space are embedded .
	manualset3
134376	3	406825	5	NULL	NULL	0	NULL	object 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several cyclic memory attractors that correspond to several simple motions of the object in two-dimensional space are embedded .
	manualset3
134377	4	406825	5	NULL	NULL	0	NULL	two-dimensional space	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several cyclic memory attractors that correspond to several simple motions of the object in two-dimensional space are embedded .
	manualset3
134378	1	406826	5	NULL	NULL	0	NULL	diarrheal stool specimens	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Several diarrheal stool specimens from the ill volunteer contained a large number of 27-nm particles .
	manualset3
134379	2	406826	5	NULL	NULL	0	NULL	ill volunteer	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Several diarrheal stool specimens from the ill volunteer contained a large number of 27-nm particles .
	manualset3
134380	3	406826	5	NULL	NULL	0	NULL	large number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several diarrheal stool specimens from the ill volunteer contained a large number of 27-nm particles .
	manualset3
134381	4	406826	5	NULL	NULL	0	NULL	27-nm particles	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Several diarrheal stool specimens from the ill volunteer contained a large number of 27-nm particles .
	manualset3
134382	1	406827	5	NULL	NULL	0	NULL	explanations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Several explanations of these counterintuitive BMI findings are discussed , as is the need for prospective research on maladaptive behavior in children and adults with this syndrome .
	manualset3
134383	2	406827	5	NULL	NULL	0	NULL	counterintuitive BMI findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Several explanations of these counterintuitive BMI findings are discussed , as is the need for prospective research on maladaptive behavior in children and adults with this syndrome .
	manualset3
134384	3	406827	5	NULL	NULL	0	NULL	prospective research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several explanations of these counterintuitive BMI findings are discussed , as is the need for prospective research on maladaptive behavior in children and adults with this syndrome .
	manualset3
134385	4	406827	5	NULL	NULL	0	NULL	maladaptive behavior	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Several explanations of these counterintuitive BMI findings are discussed , as is the need for prospective research on maladaptive behavior in children and adults with this syndrome .
	manualset3
134386	5	406827	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Several explanations of these counterintuitive BMI findings are discussed , as is the need for prospective research on maladaptive behavior in children and adults with this syndrome .
	manualset3
134387	6	406827	5	NULL	NULL	0	NULL	adults 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Several explanations of these counterintuitive BMI findings are discussed , as is the need for prospective research on maladaptive behavior in children and adults with this syndrome .
	manualset3
134388	7	406827	5	NULL	NULL	0	NULL	syndrome 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Several explanations of these counterintuitive BMI findings are discussed , as is the need for prospective research on maladaptive behavior in children and adults with this syndrome .
	manualset3
134389	1	406828	5	NULL	NULL	0	NULL	follicle cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Several follicle cells as such degenerate during previtellogenesis and their products in the form of DNA , RNA , protein and lipoprotein also seem to be absorbed directly or indirectly by the growing oocyte .
	manualset3
134390	2	406828	5	NULL	NULL	0	NULL	previtellogenesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several follicle cells as such degenerate during previtellogenesis and their products in the form of DNA , RNA , protein and lipoprotein also seem to be absorbed directly or indirectly by the growing oocyte .
	manualset3
134391	3	406828	5	NULL	NULL	0	NULL	products 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several follicle cells as such degenerate during previtellogenesis and their products in the form of DNA , RNA , protein and lipoprotein also seem to be absorbed directly or indirectly by the growing oocyte .
	manualset3
134392	4	406828	5	NULL	NULL	0	NULL	DNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Several follicle cells as such degenerate during previtellogenesis and their products in the form of DNA , RNA , protein and lipoprotein also seem to be absorbed directly or indirectly by the growing oocyte .
	manualset3
134393	5	406828	5	NULL	NULL	0	NULL	RNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Several follicle cells as such degenerate during previtellogenesis and their products in the form of DNA , RNA , protein and lipoprotein also seem to be absorbed directly or indirectly by the growing oocyte .
	manualset3
134394	6	406828	5	NULL	NULL	0	NULL	protein 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Several follicle cells as such degenerate during previtellogenesis and their products in the form of DNA , RNA , protein and lipoprotein also seem to be absorbed directly or indirectly by the growing oocyte .
	manualset3
134395	7	406828	5	NULL	NULL	0	NULL	lipoprotein 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Several follicle cells as such degenerate during previtellogenesis and their products in the form of DNA , RNA , protein and lipoprotein also seem to be absorbed directly or indirectly by the growing oocyte .
	manualset3
134396	8	406828	5	NULL	NULL	0	NULL	growing oocyte	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Several follicle cells as such degenerate during previtellogenesis and their products in the form of DNA , RNA , protein and lipoprotein also seem to be absorbed directly or indirectly by the growing oocyte .
	manualset3
134397	1	406829	5	NULL	NULL	0	NULL	independent variables	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several independent variables were related to MRSA colonization .
	manualset3
134398	2	406829	5	NULL	NULL	0	NULL	MRSA colonization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Several independent variables were related to MRSA colonization .
	manualset3
134399	1	406830	5	NULL	NULL	0	NULL	insertion or deletion events 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several insertion or deletion events were found which may have led to the specialization of each PP2C family .
	manualset3
134400	2	406830	5	NULL	NULL	0	NULL	specialization 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several insertion or deletion events were found which may have led to the specialization of each PP2C family .
	manualset3
134401	3	406830	5	NULL	NULL	0	NULL	PP2C family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Several insertion or deletion events were found which may have led to the specialization of each PP2C family .
	manualset3
134813	1	406831	5	NULL	NULL	0	NULL	note	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A note on the Winchester goose and kindred topics .
	manualset3
134814	2	406831	5	NULL	NULL	0	NULL	Winchester goose	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A note on the Winchester goose and kindred topics .
	manualset3
134815	3	406831	5	NULL	NULL	0	NULL	kindred topics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A note on the Winchester goose and kindred topics .
	manualset3
134816	1	406832	5	NULL	NULL	0	NULL	latent class analyses ( LCA )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several large-sample latent class analyses ( LCA ) have identified latent clinical and nonclinical classes of unipolar depression , but LCA is vulnerable to identification of spurious classes .
	manualset3
134817	2	406832	5	NULL	NULL	0	NULL	latent clinicalclasses of unipolar depression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Several large-sample latent class analyses ( LCA ) have identified latent clinical and nonclinical classes of unipolar depression , but LCA is vulnerable to identification of spurious classes .
	manualset3
134818	3	406832	5	NULL	NULL	0	NULL	latent nonclinical classes of unipolar depression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Several large-sample latent class analyses ( LCA ) have identified latent clinical and nonclinical classes of unipolar depression , but LCA is vulnerable to identification of spurious classes .
	manualset3
134819	4	406832	5	NULL	NULL	0	NULL	LCA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several large-sample latent class analyses ( LCA ) have identified latent clinical and nonclinical classes of unipolar depression , but LCA is vulnerable to identification of spurious classes .
	manualset3
134820	5	406832	5	NULL	NULL	0	NULL	identification	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Several large-sample latent class analyses ( LCA ) have identified latent clinical and nonclinical classes of unipolar depression , but LCA is vulnerable to identification of spurious classes .
	manualset3
134821	6	406832	5	NULL	NULL	0	NULL	spurious classes	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several large-sample latent class analyses ( LCA ) have identified latent clinical and nonclinical classes of unipolar depression , but LCA is vulnerable to identification of spurious classes .
	manualset3
134822	1	406833	5	NULL	NULL	0	NULL	lines of evidence	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence , including the detection of internal ( ( 3 ) H ) GroPIns , indicated that GroPIns is transported intact through CaGit1 .
	manualset3
134823	2	406833	5	NULL	NULL	0	NULL	detection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence , including the detection of internal ( ( 3 ) H ) GroPIns , indicated that GroPIns is transported intact through CaGit1 .
	manualset3
134824	3	406833	5	NULL	NULL	0	NULL	internal ( ( 3 ) H ) GroPIns	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence , including the detection of internal ( ( 3 ) H ) GroPIns , indicated that GroPIns is transported intact through CaGit1 .
	manualset3
134825	4	406833	5	NULL	NULL	0	NULL	GroPIns	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence , including the detection of internal ( ( 3 ) H ) GroPIns , indicated that GroPIns is transported intact through CaGit1 .
	manualset3
134826	5	406833	5	NULL	NULL	0	NULL	CaGit1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence , including the detection of internal ( ( 3 ) H ) GroPIns , indicated that GroPIns is transported intact through CaGit1 .
	manualset3
134827	1	406834	5	NULL	NULL	0	NULL	lines of evidence	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence coincide in identifying stimulatory and growth signals delivered by B-cell receptor ( BCR ) , and co-receptors together with NFkB pathway , as being the driving force in B-cell survival in CLL .
	manualset3
134828	2	406834	5	NULL	NULL	0	NULL	stimulatory signals	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence coincide in identifying stimulatory and growth signals delivered by B-cell receptor ( BCR ) , and co-receptors together with NFkB pathway , as being the driving force in B-cell survival in CLL .
	manualset3
134829	3	406834	5	NULL	NULL	0	NULL	growth signals	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence coincide in identifying stimulatory and growth signals delivered by B-cell receptor ( BCR ) , and co-receptors together with NFkB pathway , as being the driving force in B-cell survival in CLL .
	manualset3
134830	4	406834	5	NULL	NULL	0	NULL	B-cell receptor ( BCR )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence coincide in identifying stimulatory and growth signals delivered by B-cell receptor ( BCR ) , and co-receptors together with NFkB pathway , as being the driving force in B-cell survival in CLL .
	manualset3
134831	5	406834	5	NULL	NULL	0	NULL	co-receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence coincide in identifying stimulatory and growth signals delivered by B-cell receptor ( BCR ) , and co-receptors together with NFkB pathway , as being the driving force in B-cell survival in CLL .
	manualset3
134832	6	406834	5	NULL	NULL	0	NULL	NFkB pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence coincide in identifying stimulatory and growth signals delivered by B-cell receptor ( BCR ) , and co-receptors together with NFkB pathway , as being the driving force in B-cell survival in CLL .
	manualset3
134833	7	406834	5	NULL	NULL	0	NULL	driving force	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence coincide in identifying stimulatory and growth signals delivered by B-cell receptor ( BCR ) , and co-receptors together with NFkB pathway , as being the driving force in B-cell survival in CLL .
	manualset3
134834	8	406834	5	NULL	NULL	0	NULL	B-cell survival	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence coincide in identifying stimulatory and growth signals delivered by B-cell receptor ( BCR ) , and co-receptors together with NFkB pathway , as being the driving force in B-cell survival in CLL .
	manualset3
134835	9	406834	5	NULL	NULL	0	NULL	CLL 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence coincide in identifying stimulatory and growth signals delivered by B-cell receptor ( BCR ) , and co-receptors together with NFkB pathway , as being the driving force in B-cell survival in CLL .
	manualset3
134836	1	406835	5	NULL	NULL	0	NULL	lines of evidence	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence suggest the potential contribution of bacterial infection in CMV reactivation along with the potential application of CpG-ODNs in gene therapy as a stimulator for the optimal expression of target genes under the control of the CMV IE enhancer/promoter .
	manualset3
134837	2	406835	5	NULL	NULL	0	NULL	potential contribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence suggest the potential contribution of bacterial infection in CMV reactivation along with the potential application of CpG-ODNs in gene therapy as a stimulator for the optimal expression of target genes under the control of the CMV IE enhancer/promoter .
	manualset3
134838	3	406835	5	NULL	NULL	0	NULL	bacterial infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence suggest the potential contribution of bacterial infection in CMV reactivation along with the potential application of CpG-ODNs in gene therapy as a stimulator for the optimal expression of target genes under the control of the CMV IE enhancer/promoter .
	manualset3
134839	4	406835	5	NULL	NULL	0	NULL	CMV reactivation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence suggest the potential contribution of bacterial infection in CMV reactivation along with the potential application of CpG-ODNs in gene therapy as a stimulator for the optimal expression of target genes under the control of the CMV IE enhancer/promoter .
	manualset3
134840	5	406835	5	NULL	NULL	0	NULL	potential application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence suggest the potential contribution of bacterial infection in CMV reactivation along with the potential application of CpG-ODNs in gene therapy as a stimulator for the optimal expression of target genes under the control of the CMV IE enhancer/promoter .
	manualset3
134841	6	406835	5	NULL	NULL	0	NULL	CpG-ODNs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence suggest the potential contribution of bacterial infection in CMV reactivation along with the potential application of CpG-ODNs in gene therapy as a stimulator for the optimal expression of target genes under the control of the CMV IE enhancer/promoter .
	manualset3
134842	7	406835	5	NULL	NULL	0	NULL	gene therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence suggest the potential contribution of bacterial infection in CMV reactivation along with the potential application of CpG-ODNs in gene therapy as a stimulator for the optimal expression of target genes under the control of the CMV IE enhancer/promoter .
	manualset3
134843	8	406835	5	NULL	NULL	0	NULL	stimulator	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence suggest the potential contribution of bacterial infection in CMV reactivation along with the potential application of CpG-ODNs in gene therapy as a stimulator for the optimal expression of target genes under the control of the CMV IE enhancer/promoter .
	manualset3
134844	9	406835	5	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence suggest the potential contribution of bacterial infection in CMV reactivation along with the potential application of CpG-ODNs in gene therapy as a stimulator for the optimal expression of target genes under the control of the CMV IE enhancer/promoter .
	manualset3
134845	10	406835	5	NULL	NULL	0	NULL	target genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence suggest the potential contribution of bacterial infection in CMV reactivation along with the potential application of CpG-ODNs in gene therapy as a stimulator for the optimal expression of target genes under the control of the CMV IE enhancer/promoter .
	manualset3
134846	11	406835	5	NULL	NULL	0	NULL	control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence suggest the potential contribution of bacterial infection in CMV reactivation along with the potential application of CpG-ODNs in gene therapy as a stimulator for the optimal expression of target genes under the control of the CMV IE enhancer/promoter .
	manualset3
134847	12	406835	5	NULL	NULL	0	NULL	CMV IE enhancer/promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of evidence suggest the potential contribution of bacterial infection in CMV reactivation along with the potential application of CpG-ODNs in gene therapy as a stimulator for the optimal expression of target genes under the control of the CMV IE enhancer/promoter .
	manualset3
134879	1	406836	5	NULL	NULL	0	NULL	lines of research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of research have indicated that the metabolism of both RNA and protein in the brain are important for permanent learning .
	manualset3
134880	2	406836	5	NULL	NULL	0	NULL	metabolism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of research have indicated that the metabolism of both RNA and protein in the brain are important for permanent learning .
	manualset3
134881	3	406836	5	NULL	NULL	0	NULL	RNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of research have indicated that the metabolism of both RNA and protein in the brain are important for permanent learning .
	manualset3
134882	4	406836	5	NULL	NULL	0	NULL	protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of research have indicated that the metabolism of both RNA and protein in the brain are important for permanent learning .
	manualset3
134883	5	406836	5	NULL	NULL	0	NULL	brain 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of research have indicated that the metabolism of both RNA and protein in the brain are important for permanent learning .
	manualset3
134884	6	406836	5	NULL	NULL	0	NULL	permanent learning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several lines of research have indicated that the metabolism of both RNA and protein in the brain are important for permanent learning .
	manualset3
134887	1	406837	5	NULL	NULL	0	NULL	means 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Several means have now evolved and in advanced breast cancer , where the treatment may profoundly affect the patient 's sense of wellbeing , effort is being made to find out how much .
	manualset3
134893	2	406837	5	NULL	NULL	0	NULL	breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Several means have now evolved and in advanced breast cancer , where the treatment may profoundly affect the patient 's sense of wellbeing , effort is being made to find out how much .
	manualset3
134894	3	406837	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Several means have now evolved and in advanced breast cancer , where the treatment may profoundly affect the patient 's sense of wellbeing , effort is being made to find out how much .
	manualset3
134895	4	406837	5	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Several means have now evolved and in advanced breast cancer , where the treatment may profoundly affect the patient 's sense of wellbeing , effort is being made to find out how much .
	manualset3
134896	5	406837	5	NULL	NULL	0	NULL	sense of wellbeing 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several means have now evolved and in advanced breast cancer , where the treatment may profoundly affect the patient 's sense of wellbeing , effort is being made to find out how much .
	manualset3
134897	6	406837	5	NULL	NULL	0	NULL	effort 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Several means have now evolved and in advanced breast cancer , where the treatment may profoundly affect the patient 's sense of wellbeing , effort is being made to find out how much .
	manualset3
134945	1	406838	5	NULL	NULL	0	NULL	mechanisms 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Several mechanisms have been described to date , mediating the movements of different redox forms of ascorbic acid across cell membranes .
	manualset3
134946	2	406838	5	NULL	NULL	0	NULL	date 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Several mechanisms have been described to date , mediating the movements of different redox forms of ascorbic acid across cell membranes .
	manualset3
134947	3	406838	5	NULL	NULL	0	NULL	movements 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Several mechanisms have been described to date , mediating the movements of different redox forms of ascorbic acid across cell membranes .
	manualset3
134948	4	406838	5	NULL	NULL	0	NULL	redox forms of ascorbic acid	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Several mechanisms have been described to date , mediating the movements of different redox forms of ascorbic acid across cell membranes .
	manualset3
134949	5	406838	5	NULL	NULL	0	NULL	cell membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Several mechanisms have been described to date , mediating the movements of different redox forms of ascorbic acid across cell membranes .
	manualset3
135098	1	406839	5	NULL	NULL	0	NULL	mechanisms 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Several mechanisms involved in ROS generation in neurodegeneration have been proposed .
	manualset3
135099	2	406839	5	NULL	NULL	0	NULL	ROS generation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several mechanisms involved in ROS generation in neurodegeneration have been proposed .
	manualset3
135100	3	406839	5	NULL	NULL	0	NULL	neurodegeneration 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Several mechanisms involved in ROS generation in neurodegeneration have been proposed .
	manualset3
135101	1	406840	5	NULL	NULL	0	NULL	members 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several members ( 0.5 microM ) increased the accumulation of mitoxantrone ( MX ) in human breast cancer cells ( MDA-MB-231 ) transfected with ABCG2 and re-sensitized these cells to the cytotoxic effects of MX .
	manualset3
135102	2	406840	5	NULL	NULL	0	NULL	0.5 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Several members ( 0.5 microM ) increased the accumulation of mitoxantrone ( MX ) in human breast cancer cells ( MDA-MB-231 ) transfected with ABCG2 and re-sensitized these cells to the cytotoxic effects of MX .
	manualset3
135103	3	406840	5	NULL	NULL	0	NULL	accumulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several members ( 0.5 microM ) increased the accumulation of mitoxantrone ( MX ) in human breast cancer cells ( MDA-MB-231 ) transfected with ABCG2 and re-sensitized these cells to the cytotoxic effects of MX .
	manualset3
135104	4	406840	5	NULL	NULL	0	NULL	mitoxantrone ( MX ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Several members ( 0.5 microM ) increased the accumulation of mitoxantrone ( MX ) in human breast cancer cells ( MDA-MB-231 ) transfected with ABCG2 and re-sensitized these cells to the cytotoxic effects of MX .
	manualset3
135105	5	406840	5	NULL	NULL	0	NULL	human breast cancer cells ( MDA-MB-231 )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Several members ( 0.5 microM ) increased the accumulation of mitoxantrone ( MX ) in human breast cancer cells ( MDA-MB-231 ) transfected with ABCG2 and re-sensitized these cells to the cytotoxic effects of MX .
	manualset3
135106	6	406840	5	NULL	NULL	0	NULL	ABCG2 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Several members ( 0.5 microM ) increased the accumulation of mitoxantrone ( MX ) in human breast cancer cells ( MDA-MB-231 ) transfected with ABCG2 and re-sensitized these cells to the cytotoxic effects of MX .
	manualset3
135107	7	406840	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Several members ( 0.5 microM ) increased the accumulation of mitoxantrone ( MX ) in human breast cancer cells ( MDA-MB-231 ) transfected with ABCG2 and re-sensitized these cells to the cytotoxic effects of MX .
	manualset3
135108	8	406840	5	NULL	NULL	0	NULL	cytotoxic effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several members ( 0.5 microM ) increased the accumulation of mitoxantrone ( MX ) in human breast cancer cells ( MDA-MB-231 ) transfected with ABCG2 and re-sensitized these cells to the cytotoxic effects of MX .
	manualset3
135109	9	406840	5	NULL	NULL	0	NULL	MX 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Several members ( 0.5 microM ) increased the accumulation of mitoxantrone ( MX ) in human breast cancer cells ( MDA-MB-231 ) transfected with ABCG2 and re-sensitized these cells to the cytotoxic effects of MX .
	manualset3
135110	1	406841	5	NULL	NULL	0	NULL	evaluation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel , nonbinary evaluation of success and failure reveals bupropion efficacy versus methamphetamine dependence : reanalysis of a multisite trial .
	manualset3
135111	2	406841	5	NULL	NULL	0	NULL	success 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel , nonbinary evaluation of success and failure reveals bupropion efficacy versus methamphetamine dependence : reanalysis of a multisite trial .
	manualset3
135112	3	406841	5	NULL	NULL	0	NULL	failure 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel , nonbinary evaluation of success and failure reveals bupropion efficacy versus methamphetamine dependence : reanalysis of a multisite trial .
	manualset3
135113	4	406841	5	NULL	NULL	0	NULL	bupropion efficacy	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel , nonbinary evaluation of success and failure reveals bupropion efficacy versus methamphetamine dependence : reanalysis of a multisite trial .
	manualset3
135114	5	406841	5	NULL	NULL	0	NULL	methamphetamine dependence	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel , nonbinary evaluation of success and failure reveals bupropion efficacy versus methamphetamine dependence : reanalysis of a multisite trial .
	manualset3
135115	6	406841	5	NULL	NULL	0	NULL	reanalysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel , nonbinary evaluation of success and failure reveals bupropion efficacy versus methamphetamine dependence : reanalysis of a multisite trial .
	manualset3
135116	7	406841	5	NULL	NULL	NULL	NULL	multisite trial	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A novel , nonbinary evaluation of success and failure reveals bupropion efficacy versus methamphetamine dependence : reanalysis of a multisite trial .
	manualset3
135117	1	406842	5	NULL	NULL	0	NULL	methods 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Several methods have been developed for VIIIR : Ag evaluation , among the first being the rocket-immunoelectrophoresis method of LAURELL .
	manualset3
135118	2	406842	5	NULL	NULL	0	NULL	VIIIR : Ag evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several methods have been developed for VIIIR : Ag evaluation , among the first being the rocket-immunoelectrophoresis method of LAURELL .
	manualset3
135119	3	406842	5	NULL	NULL	0	NULL	rocket-immunoelectrophoresis method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several methods have been developed for VIIIR : Ag evaluation , among the first being the rocket-immunoelectrophoresis method of LAURELL .
	manualset3
135120	4	406842	5	NULL	NULL	0	NULL	LAURELL	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Several methods have been developed for VIIIR : Ag evaluation , among the first being the rocket-immunoelectrophoresis method of LAURELL .
	manualset3
135121	1	406843	5	NULL	NULL	0	NULL	mouse central nervous system genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Several mouse central nervous system genes have been identified that are differentially regulated during Japanese encephalitis virus ( JEV ) infection , including those which have not been reported to be induced by any other neurotropic virus .
	manualset3
135122	2	406843	5	NULL	NULL	0	NULL	Japanese encephalitis virus ( JEV ) infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Several mouse central nervous system genes have been identified that are differentially regulated during Japanese encephalitis virus ( JEV ) infection , including those which have not been reported to be induced by any other neurotropic virus .
	manualset3
135123	3	406843	5	NULL	NULL	0	NULL	neurotropic virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Several mouse central nervous system genes have been identified that are differentially regulated during Japanese encephalitis virus ( JEV ) infection , including those which have not been reported to be induced by any other neurotropic virus .
	manualset3
135124	1	406844	5	NULL	NULL	0	NULL	mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several mutations that removed C-type inactivation also made the channels resistant to becoming defunct .
	manualset3
135125	2	406844	5	NULL	NULL	0	NULL	C-type inactivation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several mutations that removed C-type inactivation also made the channels resistant to becoming defunct .
	manualset3
135126	3	406844	5	NULL	NULL	0	NULL	channels 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Several mutations that removed C-type inactivation also made the channels resistant to becoming defunct .
	manualset3
135127	1	406845	5	NULL	NULL	0	NULL	 novel algorithms	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Several novel algorithms are brought together in this tool : the tba multisequence aligner program used to rapidly identify local sequence conservation and the multiTF program to detect evolutionarily conserved transcription factor binding sites in alignments .
	manualset3
135128	2	406845	5	NULL	NULL	0	NULL	tool 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Several novel algorithms are brought together in this tool : the tba multisequence aligner program used to rapidly identify local sequence conservation and the multiTF program to detect evolutionarily conserved transcription factor binding sites in alignments .
	manualset3
135129	3	406845	5	NULL	NULL	0	NULL	tba multisequence aligner program 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Several novel algorithms are brought together in this tool : the tba multisequence aligner program used to rapidly identify local sequence conservation and the multiTF program to detect evolutionarily conserved transcription factor binding sites in alignments .
	manualset3
135130	4	406845	5	NULL	NULL	0	NULL	local sequence conservation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several novel algorithms are brought together in this tool : the tba multisequence aligner program used to rapidly identify local sequence conservation and the multiTF program to detect evolutionarily conserved transcription factor binding sites in alignments .
	manualset3
135131	5	406845	5	NULL	NULL	0	NULL	multiTF program	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Several novel algorithms are brought together in this tool : the tba multisequence aligner program used to rapidly identify local sequence conservation and the multiTF program to detect evolutionarily conserved transcription factor binding sites in alignments .
	manualset3
135132	6	406845	5	NULL	NULL	0	NULL	evolutionarily conserved transcription factor binding sites	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Several novel algorithms are brought together in this tool : the tba multisequence aligner program used to rapidly identify local sequence conservation and the multiTF program to detect evolutionarily conserved transcription factor binding sites in alignments .
	manualset3
135133	7	406845	5	NULL	NULL	0	NULL	alignments 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several novel algorithms are brought together in this tool : the tba multisequence aligner program used to rapidly identify local sequence conservation and the multiTF program to detect evolutionarily conserved transcription factor binding sites in alignments .
	manualset3
135134	1	406846	5	NULL	NULL	0	NULL	elements 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several of these elements were combined to calculate Quality Control , Screening Utility , and Surveillance Utility scores for each standard .
	manualset3
135135	2	406846	5	NULL	NULL	NULL	NULL	Quality Control scores 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Several of these elements were combined to calculate Quality Control , Screening Utility , and Surveillance Utility scores for each standard .
	manualset3
135136	3	406846	5	NULL	NULL	0	NULL	Screening Utility scores 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several of these elements were combined to calculate Quality Control , Screening Utility , and Surveillance Utility scores for each standard .
	manualset3
135137	4	406846	5	NULL	NULL	0	NULL	Surveillance Utility scores	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several of these elements were combined to calculate Quality Control , Screening Utility , and Surveillance Utility scores for each standard .
	manualset3
135138	5	406846	5	NULL	NULL	0	NULL	standard 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several of these elements were combined to calculate Quality Control , Screening Utility , and Surveillance Utility scores for each standard .
	manualset3
135139	1	406847	5	NULL	NULL	0	NULL	pathways 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several pathways of drug metabolizing enzymic activity were measured in hepatic fractions of the channel catfish and rat using model substrates .
	manualset3
135140	2	406847	5	NULL	NULL	0	NULL	drug metabolizing enzymic activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several pathways of drug metabolizing enzymic activity were measured in hepatic fractions of the channel catfish and rat using model substrates .
	manualset3
135141	3	406847	5	NULL	NULL	0	NULL	hepatic fractions	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Several pathways of drug metabolizing enzymic activity were measured in hepatic fractions of the channel catfish and rat using model substrates .
	manualset3
135142	4	406847	5	NULL	NULL	0	NULL	channel catfish	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Several pathways of drug metabolizing enzymic activity were measured in hepatic fractions of the channel catfish and rat using model substrates .
	manualset3
135143	5	406847	5	NULL	NULL	0	NULL	rat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Several pathways of drug metabolizing enzymic activity were measured in hepatic fractions of the channel catfish and rat using model substrates .
	manualset3
135144	6	406847	5	NULL	NULL	0	NULL	model substrates	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Several pathways of drug metabolizing enzymic activity were measured in hepatic fractions of the channel catfish and rat using model substrates .
	manualset3
135145	1	406848	5	NULL	NULL	0	NULL	potential ERK consensus sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Several potential ERK consensus sites within the C-terminal region of SAP1a can modulate its transactivation efficacy , implicating that SAP1a is a direct target of ERKs .
	manualset3
135146	2	406848	5	NULL	NULL	0	NULL	C-terminal region of SAP1a	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Several potential ERK consensus sites within the C-terminal region of SAP1a can modulate its transactivation efficacy , implicating that SAP1a is a direct target of ERKs .
	manualset3
135147	3	406848	5	NULL	NULL	0	NULL	transactivation efficacy	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several potential ERK consensus sites within the C-terminal region of SAP1a can modulate its transactivation efficacy , implicating that SAP1a is a direct target of ERKs .
	manualset3
135148	4	406848	5	NULL	NULL	0	NULL	SAP1a 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Several potential ERK consensus sites within the C-terminal region of SAP1a can modulate its transactivation efficacy , implicating that SAP1a is a direct target of ERKs .
	manualset3
135149	5	406848	5	NULL	NULL	0	NULL	direct target	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Several potential ERK consensus sites within the C-terminal region of SAP1a can modulate its transactivation efficacy , implicating that SAP1a is a direct target of ERKs .
	manualset3
135150	6	406848	5	NULL	NULL	0	NULL	ERKs 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Several potential ERK consensus sites within the C-terminal region of SAP1a can modulate its transactivation efficacy , implicating that SAP1a is a direct target of ERKs .
	manualset3
135151	1	406849	5	NULL	NULL	0	NULL	proteases 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Several proteases , including Neutral protease from Bacillus polymyxa , were found to release N - ( 1-deoxyfructosyl ) - Val-His efficiently , however no protease was found to release N - ( 1-deoxyfructosyl ) - Val .
	manualset3
135152	2	406849	5	NULL	NULL	0	NULL	Neutral protease 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Several proteases , including Neutral protease from Bacillus polymyxa , were found to release N - ( 1-deoxyfructosyl ) - Val-His efficiently , however no protease was found to release N - ( 1-deoxyfructosyl ) - Val .
	manualset3
135153	3	406849	5	NULL	NULL	0	NULL	Bacillus polymyxa	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Several proteases , including Neutral protease from Bacillus polymyxa , were found to release N - ( 1-deoxyfructosyl ) - Val-His efficiently , however no protease was found to release N - ( 1-deoxyfructosyl ) - Val .
	manualset3
135154	4	406849	5	NULL	NULL	0	NULL	N - ( 1-deoxyfructosyl ) - Val-His	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Several proteases , including Neutral protease from Bacillus polymyxa , were found to release N - ( 1-deoxyfructosyl ) - Val-His efficiently , however no protease was found to release N - ( 1-deoxyfructosyl ) - Val .
	manualset3
135155	5	406849	5	NULL	NULL	0	NULL	protease 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Several proteases , including Neutral protease from Bacillus polymyxa , were found to release N - ( 1-deoxyfructosyl ) - Val-His efficiently , however no protease was found to release N - ( 1-deoxyfructosyl ) - Val .
	manualset3
135156	6	406849	5	NULL	NULL	0	NULL	N - ( 1-deoxyfructosyl ) - Val	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Several proteases , including Neutral protease from Bacillus polymyxa , were found to release N - ( 1-deoxyfructosyl ) - Val-His efficiently , however no protease was found to release N - ( 1-deoxyfructosyl ) - Val .
	manualset3
135157	1	406850	5	NULL	NULL	0	NULL	reports 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Several recent reports have established that the primary function of HR enzymes is to underpin DNA replication , resetting forks that are blocked or collapsed at sites of DNA damage remote from replication origins .
	manualset3
135158	2	406850	5	NULL	NULL	0	NULL	primary function 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several recent reports have established that the primary function of HR enzymes is to underpin DNA replication , resetting forks that are blocked or collapsed at sites of DNA damage remote from replication origins .
	manualset3
135159	3	406850	5	NULL	NULL	0	NULL	HR enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Several recent reports have established that the primary function of HR enzymes is to underpin DNA replication , resetting forks that are blocked or collapsed at sites of DNA damage remote from replication origins .
	manualset3
135160	4	406850	5	NULL	NULL	0	NULL	DNA replication	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several recent reports have established that the primary function of HR enzymes is to underpin DNA replication , resetting forks that are blocked or collapsed at sites of DNA damage remote from replication origins .
	manualset3
135161	5	406850	5	NULL	NULL	0	NULL	forks 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Several recent reports have established that the primary function of HR enzymes is to underpin DNA replication , resetting forks that are blocked or collapsed at sites of DNA damage remote from replication origins .
	manualset3
135162	6	406850	5	NULL	NULL	0	NULL	sites of DNA damage	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Several recent reports have established that the primary function of HR enzymes is to underpin DNA replication , resetting forks that are blocked or collapsed at sites of DNA damage remote from replication origins .
	manualset3
135163	7	406850	5	NULL	NULL	0	NULL	replication origins	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Several recent reports have established that the primary function of HR enzymes is to underpin DNA replication , resetting forks that are blocked or collapsed at sites of DNA damage remote from replication origins .
	manualset3
135164	1	406851	5	NULL	NULL	0	NULL	 risk factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several risk factors predispose to atherosclerosis including hypertension and abnormalities in lipoprotein metabolism and glucose homeostasis .
	manualset3
135165	2	406851	5	NULL	NULL	0	NULL	atherosclerosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Several risk factors predispose to atherosclerosis including hypertension and abnormalities in lipoprotein metabolism and glucose homeostasis .
	manualset3
135166	3	406851	5	NULL	NULL	0	NULL	hypertension 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Several risk factors predispose to atherosclerosis including hypertension and abnormalities in lipoprotein metabolism and glucose homeostasis .
	manualset3
135167	4	406851	5	NULL	NULL	0	NULL	abnormalities in lipoprotein metabolism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Several risk factors predispose to atherosclerosis including hypertension and abnormalities in lipoprotein metabolism and glucose homeostasis .
	manualset3
135168	5	406851	5	NULL	NULL	0	NULL	abnormalities in glucose homeostasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Several risk factors predispose to atherosclerosis including hypertension and abnormalities in lipoprotein metabolism and glucose homeostasis .
	manualset3
135169	1	406852	5	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several studies currently under way may help to increase the effectiveness and dissemination of office-based tobacco cessation programs into routine dental care .
	manualset3
135170	2	406852	5	NULL	NULL	0	NULL	effectiveness 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Several studies currently under way may help to increase the effectiveness and dissemination of office-based tobacco cessation programs into routine dental care .
	manualset3
135171	3	406852	5	NULL	NULL	0	NULL	dissemination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Several studies currently under way may help to increase the effectiveness and dissemination of office-based tobacco cessation programs into routine dental care .
	manualset3
135172	4	406852	5	NULL	NULL	NULL	NULL	office-based tobacco cessation programs	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Several studies currently under way may help to increase the effectiveness and dissemination of office-based tobacco cessation programs into routine dental care .
	manualset3
135173	5	406852	5	NULL	NULL	0	NULL	routine dental care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Several studies currently under way may help to increase the effectiveness and dissemination of office-based tobacco cessation programs into routine dental care .
	manualset3
135174	1	406853	5	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several studies have proven that the status of the EGFR can be both an indicator of suitability for treatment with , and predict the likelihood of response to EGFR targeted therapy .
	manualset3
135175	2	406853	5	NULL	NULL	0	NULL	status 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Several studies have proven that the status of the EGFR can be both an indicator of suitability for treatment with , and predict the likelihood of response to EGFR targeted therapy .
	manualset3
135176	3	406853	5	NULL	NULL	0	NULL	EGFR 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Several studies have proven that the status of the EGFR can be both an indicator of suitability for treatment with , and predict the likelihood of response to EGFR targeted therapy .
	manualset3
135177	4	406853	5	NULL	NULL	0	NULL	indicator 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several studies have proven that the status of the EGFR can be both an indicator of suitability for treatment with , and predict the likelihood of response to EGFR targeted therapy .
	manualset3
135178	5	406853	5	NULL	NULL	NULL	NULL	treatment 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Several studies have proven that the status of the EGFR can be both an indicator of suitability for treatment with , and predict the likelihood of response to EGFR targeted therapy .
	manualset3
135179	6	406853	5	NULL	NULL	0	NULL	likelihood 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Several studies have proven that the status of the EGFR can be both an indicator of suitability for treatment with , and predict the likelihood of response to EGFR targeted therapy .
	manualset3
135180	7	406853	5	NULL	NULL	0	NULL	response 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several studies have proven that the status of the EGFR can be both an indicator of suitability for treatment with , and predict the likelihood of response to EGFR targeted therapy .
	manualset3
135181	8	406853	5	NULL	NULL	0	NULL	EGFR targeted therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Several studies have proven that the status of the EGFR can be both an indicator of suitability for treatment with , and predict the likelihood of response to EGFR targeted therapy .
	manualset3
138426	9	406853	5	NULL	NULL	0	NULL	suitability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Several studies have proven that the status of the EGFR can be both an indicator of suitability for treatment with , and predict the likelihood of response to EGFR targeted therapy .
	manualset3
135182	1	406854	5	NULL	NULL	0	NULL	 novel , specific binding protein assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel , specific binding protein assay for quantitation of intracellular inositol 1 , 3 , 4 , 5-tetrakisphosphate ( InsP4 ) using a high-affinity InsP4 receptor from cerebellum .
	manualset3
135183	2	406854	5	NULL	NULL	0	NULL	quantitation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel , specific binding protein assay for quantitation of intracellular inositol 1 , 3 , 4 , 5-tetrakisphosphate ( InsP4 ) using a high-affinity InsP4 receptor from cerebellum .
	manualset3
135184	3	406854	5	NULL	NULL	0	NULL	intracellular inositol 1 , 3 , 4 , 5-tetrakisphosphate ( InsP4 ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel , specific binding protein assay for quantitation of intracellular inositol 1 , 3 , 4 , 5-tetrakisphosphate ( InsP4 ) using a high-affinity InsP4 receptor from cerebellum .
	manualset3
135185	4	406854	5	NULL	NULL	0	NULL	high-affinity InsP4 receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel , specific binding protein assay for quantitation of intracellular inositol 1 , 3 , 4 , 5-tetrakisphosphate ( InsP4 ) using a high-affinity InsP4 receptor from cerebellum .
	manualset3
135186	5	406854	5	NULL	NULL	0	NULL	cerebellum 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel , specific binding protein assay for quantitation of intracellular inositol 1 , 3 , 4 , 5-tetrakisphosphate ( InsP4 ) using a high-affinity InsP4 receptor from cerebellum .
	manualset3
135187	1	406855	5	NULL	NULL	0	NULL	surveys 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several surveys were conducted in this country before and after the introduction of the new system to evaluate its impact on training and patient care .
	manualset3
135188	2	406855	5	NULL	NULL	0	NULL	country 	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Several surveys were conducted in this country before and after the introduction of the new system to evaluate its impact on training and patient care .
	manualset3
135189	3	406855	5	NULL	NULL	0	NULL	introduction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Several surveys were conducted in this country before and after the introduction of the new system to evaluate its impact on training and patient care .
	manualset3
135190	4	406855	5	NULL	NULL	0	NULL	new system	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several surveys were conducted in this country before and after the introduction of the new system to evaluate its impact on training and patient care .
	manualset3
135191	5	406855	5	NULL	NULL	0	NULL	impact 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Several surveys were conducted in this country before and after the introduction of the new system to evaluate its impact on training and patient care .
	manualset3
135192	6	406855	5	NULL	NULL	0	NULL	training 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Several surveys were conducted in this country before and after the introduction of the new system to evaluate its impact on training and patient care .
	manualset3
135193	7	406855	5	NULL	NULL	0	NULL	patient care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Several surveys were conducted in this country before and after the introduction of the new system to evaluate its impact on training and patient care .
	manualset3
135194	1	406856	5	NULL	NULL	0	NULL	systems for zinc homeostasis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several systems for zinc homeostasis have been characterized in the freshwater species Synechococcus sp .
	manualset3
135195	2	406856	5	NULL	NULL	0	NULL	freshwater species Synechococcus sp	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Several systems for zinc homeostasis have been characterized in the freshwater species Synechococcus sp .
	manualset3
135196	1	406857	5	NULL	NULL	0	NULL	thiols 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Several thiols and disulphides have been found able both to shorten the latency phase and to increase the growth of several virus strains in cell cultures .
	manualset3
135197	2	406857	5	NULL	NULL	0	NULL	disulphides 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Several thiols and disulphides have been found able both to shorten the latency phase and to increase the growth of several virus strains in cell cultures .
	manualset3
135198	3	406857	5	NULL	NULL	0	NULL	latency phase 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Several thiols and disulphides have been found able both to shorten the latency phase and to increase the growth of several virus strains in cell cultures .
	manualset3
135200	5	406857	5	NULL	NULL	0	NULL	growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several thiols and disulphides have been found able both to shorten the latency phase and to increase the growth of several virus strains in cell cultures .
	manualset3
135201	6	406857	5	NULL	NULL	0	NULL	virus strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Several thiols and disulphides have been found able both to shorten the latency phase and to increase the growth of several virus strains in cell cultures .
	manualset3
135202	7	406857	5	NULL	NULL	0	NULL	cell cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Several thiols and disulphides have been found able both to shorten the latency phase and to increase the growth of several virus strains in cell cultures .
	manualset3
135203	1	406858	5	NULL	NULL	0	NULL	types 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several types of reliability and validity testing are defined , and an easy-to-use check sheet is provided for research purposes .
	manualset3
135204	2	406858	5	NULL	NULL	0	NULL	reliability testing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several types of reliability and validity testing are defined , and an easy-to-use check sheet is provided for research purposes .
	manualset3
135205	3	406858	5	NULL	NULL	0	NULL	validity testing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several types of reliability and validity testing are defined , and an easy-to-use check sheet is provided for research purposes .
	manualset3
135206	4	406858	5	NULL	NULL	0	NULL	check sheet	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Several types of reliability and validity testing are defined , and an easy-to-use check sheet is provided for research purposes .
	manualset3
135207	5	406858	5	NULL	NULL	0	NULL	research purposes	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several types of reliability and validity testing are defined , and an easy-to-use check sheet is provided for research purposes .
	manualset3
135208	1	406859	5	NULL	NULL	0	NULL	versions 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several versions of split green fluorescent protein ( GFP ) fold and reconstitute fluorescence , as do many circular permutants , but little is known about the dependence of reconstitution on circular permutation .
	manualset3
135209	2	406859	5	NULL	NULL	0	NULL	split green fluorescent protein ( GFP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Several versions of split green fluorescent protein ( GFP ) fold and reconstitute fluorescence , as do many circular permutants , but little is known about the dependence of reconstitution on circular permutation .
	manualset3
135210	3	406859	5	NULL	NULL	0	NULL	fluorescence 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several versions of split green fluorescent protein ( GFP ) fold and reconstitute fluorescence , as do many circular permutants , but little is known about the dependence of reconstitution on circular permutation .
	manualset3
135211	4	406859	5	NULL	NULL	0	NULL	circular permutants	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Several versions of split green fluorescent protein ( GFP ) fold and reconstitute fluorescence , as do many circular permutants , but little is known about the dependence of reconstitution on circular permutation .
	manualset3
135212	5	406859	5	NULL	NULL	0	NULL	dependence 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several versions of split green fluorescent protein ( GFP ) fold and reconstitute fluorescence , as do many circular permutants , but little is known about the dependence of reconstitution on circular permutation .
	manualset3
135213	6	406859	5	NULL	NULL	0	NULL	reconstitution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Several versions of split green fluorescent protein ( GFP ) fold and reconstitute fluorescence , as do many circular permutants , but little is known about the dependence of reconstitution on circular permutation .
	manualset3
135214	7	406859	5	NULL	NULL	0	NULL	circular permutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several versions of split green fluorescent protein ( GFP ) fold and reconstitute fluorescence , as do many circular permutants , but little is known about the dependence of reconstitution on circular permutation .
	manualset3
135215	1	406860	5	NULL	NULL	0	NULL	viruses 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Several viruses encode factors that promote host mRNA degradation to silence gene expression .
	manualset3
135216	2	406860	5	NULL	NULL	NULL	NULL	factors 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Several viruses encode factors that promote host mRNA degradation to silence gene expression .
	manualset3
135217	3	406860	5	NULL	NULL	0	NULL	host mRNA degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several viruses encode factors that promote host mRNA degradation to silence gene expression .
	manualset3
135218	4	406860	5	NULL	NULL	0	NULL	gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several viruses encode factors that promote host mRNA degradation to silence gene expression .
	manualset3
135219	1	406861	5	NULL	NULL	0	NULL	Severe CI	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe CI is a characteristic of 20-47 % of individuals with apparent CFS and/or fibromyalgia , all patients with multiple chemical sensitivity ( MCS ) , and approximately 4-6 % of the general population .
	manualset3
135220	2	406861	5	NULL	NULL	0	NULL	20-47 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe CI is a characteristic of 20-47 % of individuals with apparent CFS and/or fibromyalgia , all patients with multiple chemical sensitivity ( MCS ) , and approximately 4-6 % of the general population .
	manualset3
135221	3	406861	5	NULL	NULL	0	NULL	individuals 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe CI is a characteristic of 20-47 % of individuals with apparent CFS and/or fibromyalgia , all patients with multiple chemical sensitivity ( MCS ) , and approximately 4-6 % of the general population .
	manualset3
135222	4	406861	5	NULL	NULL	0	NULL	CFS 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe CI is a characteristic of 20-47 % of individuals with apparent CFS and/or fibromyalgia , all patients with multiple chemical sensitivity ( MCS ) , and approximately 4-6 % of the general population .
	manualset3
135223	5	406861	5	NULL	NULL	0	NULL	fibromyalgia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe CI is a characteristic of 20-47 % of individuals with apparent CFS and/or fibromyalgia , all patients with multiple chemical sensitivity ( MCS ) , and approximately 4-6 % of the general population .
	manualset3
135224	6	406861	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe CI is a characteristic of 20-47 % of individuals with apparent CFS and/or fibromyalgia , all patients with multiple chemical sensitivity ( MCS ) , and approximately 4-6 % of the general population .
	manualset3
135225	7	406861	5	NULL	NULL	0	NULL	multiple chemical sensitivity ( MCS )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe CI is a characteristic of 20-47 % of individuals with apparent CFS and/or fibromyalgia , all patients with multiple chemical sensitivity ( MCS ) , and approximately 4-6 % of the general population .
	manualset3
135226	8	406861	5	NULL	NULL	0	NULL	 4-6 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe CI is a characteristic of 20-47 % of individuals with apparent CFS and/or fibromyalgia , all patients with multiple chemical sensitivity ( MCS ) , and approximately 4-6 % of the general population .
	manualset3
135227	9	406861	5	NULL	NULL	0	NULL	general population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe CI is a characteristic of 20-47 % of individuals with apparent CFS and/or fibromyalgia , all patients with multiple chemical sensitivity ( MCS ) , and approximately 4-6 % of the general population .
	manualset3
135228	1	406862	5	NULL	NULL	0	NULL	CEM 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel CEM enhanced EK method with approaching anodes ( AAs ) is proposed to accelerate electro-migration effect .
	manualset3
135229	2	406862	5	NULL	NULL	0	NULL	EK method	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel CEM enhanced EK method with approaching anodes ( AAs ) is proposed to accelerate electro-migration effect .
	manualset3
135230	3	406862	5	NULL	NULL	0	NULL	anodes ( AAs ) 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel CEM enhanced EK method with approaching anodes ( AAs ) is proposed to accelerate electro-migration effect .
	manualset3
135231	4	406862	5	NULL	NULL	0	NULL	electro-migration effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel CEM enhanced EK method with approaching anodes ( AAs ) is proposed to accelerate electro-migration effect .
	manualset3
135232	1	406863	5	NULL	NULL	NULL	NULL	Severe acute respiratory syndrome coronavirus protein 6	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Severe acute respiratory syndrome coronavirus protein 6 accelerates murine coronavirus infections .
	manualset3
135233	2	406863	5	NULL	NULL	0	NULL	murine coronavirus infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe acute respiratory syndrome coronavirus protein 6 accelerates murine coronavirus infections .
	manualset3
135234	1	406864	5	NULL	NULL	0	NULL	clinical courses	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe clinical courses are more frequent in non-menstrual TSS : the mortality is about 8 % -11 % in non-menstrual TSS compared to 2 % -5 % in menstrual TSS .
	manualset3
135235	2	406864	5	NULL	NULL	0	NULL	non-menstrual TSS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe clinical courses are more frequent in non-menstrual TSS : the mortality is about 8 % -11 % in non-menstrual TSS compared to 2 % -5 % in menstrual TSS .
	manualset3
135236	3	406864	5	NULL	NULL	0	NULL	mortality 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe clinical courses are more frequent in non-menstrual TSS : the mortality is about 8 % -11 % in non-menstrual TSS compared to 2 % -5 % in menstrual TSS .
	manualset3
135237	4	406864	5	NULL	NULL	0	NULL	8 % -11 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe clinical courses are more frequent in non-menstrual TSS : the mortality is about 8 % -11 % in non-menstrual TSS compared to 2 % -5 % in menstrual TSS .
	manualset3
135238	5	406864	5	NULL	NULL	0	NULL	non-menstrual TSS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe clinical courses are more frequent in non-menstrual TSS : the mortality is about 8 % -11 % in non-menstrual TSS compared to 2 % -5 % in menstrual TSS .
	manualset3
135239	6	406864	5	NULL	NULL	0	NULL	2 % -5 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe clinical courses are more frequent in non-menstrual TSS : the mortality is about 8 % -11 % in non-menstrual TSS compared to 2 % -5 % in menstrual TSS .
	manualset3
135240	7	406864	5	NULL	NULL	0	NULL	menstrual TSS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe clinical courses are more frequent in non-menstrual TSS : the mortality is about 8 % -11 % in non-menstrual TSS compared to 2 % -5 % in menstrual TSS .
	manualset3
135241	1	406865	5	NULL	NULL	0	NULL	hypercholesterolemia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe hypercholesterolemia and atherosclerosis in apolipoprotein E-deficient mice created by homologous recombination in ES cells .
	manualset3
135242	2	406865	5	NULL	NULL	0	NULL	atherosclerosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe hypercholesterolemia and atherosclerosis in apolipoprotein E-deficient mice created by homologous recombination in ES cells .
	manualset3
135243	3	406865	5	NULL	NULL	0	NULL	apolipoprotein E-deficient mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe hypercholesterolemia and atherosclerosis in apolipoprotein E-deficient mice created by homologous recombination in ES cells .
	manualset3
135244	4	406865	5	NULL	NULL	0	NULL	homologous recombination 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe hypercholesterolemia and atherosclerosis in apolipoprotein E-deficient mice created by homologous recombination in ES cells .
	manualset3
135245	5	406865	5	NULL	NULL	0	NULL	ES cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe hypercholesterolemia and atherosclerosis in apolipoprotein E-deficient mice created by homologous recombination in ES cells .
	manualset3
135246	1	406866	5	NULL	NULL	0	NULL	hypertriglyceridemia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe hypertriglyceridemia as a result of familial chylomicronemia : the Cape Town experience .
	manualset3
135247	2	406866	5	NULL	NULL	0	NULL	result 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe hypertriglyceridemia as a result of familial chylomicronemia : the Cape Town experience .
	manualset3
135248	3	406866	5	NULL	NULL	0	NULL	familial chylomicronemia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe hypertriglyceridemia as a result of familial chylomicronemia : the Cape Town experience .
	manualset3
135249	4	406866	5	NULL	NULL	0	NULL	Cape Town experience 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe hypertriglyceridemia as a result of familial chylomicronemia : the Cape Town experience .
	manualset3
135250	1	406867	5	NULL	NULL	0	NULL	paravalvular mitral regurgitation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe paravalvular mitral regurgitation is a rare but important complication of mitral valve replacement , often producing symptoms associated with refractory heart failure or hemolysis .
	manualset3
135251	2	406867	5	NULL	NULL	0	NULL	complication 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe paravalvular mitral regurgitation is a rare but important complication of mitral valve replacement , often producing symptoms associated with refractory heart failure or hemolysis .
	manualset3
135252	3	406867	5	NULL	NULL	0	NULL	mitral valve replacement	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe paravalvular mitral regurgitation is a rare but important complication of mitral valve replacement , often producing symptoms associated with refractory heart failure or hemolysis .
	manualset3
135253	4	406867	5	NULL	NULL	0	NULL	symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe paravalvular mitral regurgitation is a rare but important complication of mitral valve replacement , often producing symptoms associated with refractory heart failure or hemolysis .
	manualset3
135254	5	406867	5	NULL	NULL	0	NULL	refractory heart failure or hemolysis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe paravalvular mitral regurgitation is a rare but important complication of mitral valve replacement , often producing symptoms associated with refractory heart failure or hemolysis .
	manualset3
135255	1	406868	5	NULL	NULL	0	NULL	refeeding hypophosphatemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe refeeding hypophosphatemia in a CAPD patient : a case report .
	manualset3
135256	2	406868	5	NULL	NULL	0	NULL	CAPD patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe refeeding hypophosphatemia in a CAPD patient : a case report .
	manualset3
135257	3	406868	5	NULL	NULL	0	NULL	case report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe refeeding hypophosphatemia in a CAPD patient : a case report .
	manualset3
135258	1	406869	5	NULL	NULL	0	NULL	side effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe side effects were not noted except in 10 cases with narrowness of hepatic artery and cases of 2 biloma in patients undergoing therapy two or more times .
	manualset3
135259	2	406869	5	NULL	NULL	0	NULL	10 cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe side effects were not noted except in 10 cases with narrowness of hepatic artery and cases of 2 biloma in patients undergoing therapy two or more times .
	manualset3
135260	3	406869	5	NULL	NULL	0	NULL	hepatic artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe side effects were not noted except in 10 cases with narrowness of hepatic artery and cases of 2 biloma in patients undergoing therapy two or more times .
	manualset3
135261	4	406869	5	NULL	NULL	0	NULL	cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe side effects were not noted except in 10 cases with narrowness of hepatic artery and cases of 2 biloma in patients undergoing therapy two or more times .
	manualset3
135262	5	406869	5	NULL	NULL	0	NULL	2 biloma 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe side effects were not noted except in 10 cases with narrowness of hepatic artery and cases of 2 biloma in patients undergoing therapy two or more times .
	manualset3
135263	6	406869	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe side effects were not noted except in 10 cases with narrowness of hepatic artery and cases of 2 biloma in patients undergoing therapy two or more times .
	manualset3
135264	7	406869	5	NULL	NULL	0	NULL	therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe side effects were not noted except in 10 cases with narrowness of hepatic artery and cases of 2 biloma in patients undergoing therapy two or more times .
	manualset3
135265	8	406869	5	NULL	NULL	0	NULL	two or more times	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Severe side effects were not noted except in 10 cases with narrowness of hepatic artery and cases of 2 biloma in patients undergoing therapy two or more times .
	manualset3
135266	1	406870	5	NULL	NULL	0	NULL	Severin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Severin from Dictyostelium discoideum is a Ca2 ( + ) - activated actin-binding protein that severs actin filaments , nucleates actin assembly , and caps the fast growing ends of actin filaments .
	manualset3
135267	2	406870	5	NULL	NULL	0	NULL	Dictyostelium discoideum 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Severin from Dictyostelium discoideum is a Ca2 ( + ) - activated actin-binding protein that severs actin filaments , nucleates actin assembly , and caps the fast growing ends of actin filaments .
	manualset3
135268	3	406870	5	NULL	NULL	0	NULL	Ca2 ( + ) - activated actin-binding protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Severin from Dictyostelium discoideum is a Ca2 ( + ) - activated actin-binding protein that severs actin filaments , nucleates actin assembly , and caps the fast growing ends of actin filaments .
	manualset3
135269	4	406870	5	NULL	NULL	0	NULL	actin filaments 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Severin from Dictyostelium discoideum is a Ca2 ( + ) - activated actin-binding protein that severs actin filaments , nucleates actin assembly , and caps the fast growing ends of actin filaments .
	manualset3
135270	5	406870	5	NULL	NULL	0	NULL	actin assembly	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Severin from Dictyostelium discoideum is a Ca2 ( + ) - activated actin-binding protein that severs actin filaments , nucleates actin assembly , and caps the fast growing ends of actin filaments .
	manualset3
135271	6	406870	5	NULL	NULL	NULL	NULL	fast growing ends	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Severin from Dictyostelium discoideum is a Ca2 ( + ) - activated actin-binding protein that severs actin filaments , nucleates actin assembly , and caps the fast growing ends of actin filaments .
	manualset3
135272	7	406870	5	NULL	NULL	0	NULL	actin filaments	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Severin from Dictyostelium discoideum is a Ca2 ( + ) - activated actin-binding protein that severs actin filaments , nucleates actin assembly , and caps the fast growing ends of actin filaments .
	manualset3
135273	1	406871	5	NULL	NULL	0	NULL	Sex-specific heritability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex-specific heritability of cell-mediated immune response in the blue tit nestlings ( Cyanistes caeruleus ) .
	manualset3
135274	2	406871	5	NULL	NULL	0	NULL	cell-mediated immune response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex-specific heritability of cell-mediated immune response in the blue tit nestlings ( Cyanistes caeruleus ) .
	manualset3
135275	3	406871	5	NULL	NULL	0	NULL	blue tit nestlings ( Cyanistes caeruleus ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex-specific heritability of cell-mediated immune response in the blue tit nestlings ( Cyanistes caeruleus ) .
	manualset3
135276	1	406872	5	NULL	NULL	0	NULL	NKG2-specific mAb ( termed P25 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel NKG2-specific mAb ( termed P25 ) has been generated that specifically reacts with both NKG2-A and NKG2-C molecules , but fails to recognize NKG2-E molecules .
	manualset3
135277	2	406872	5	NULL	NULL	0	NULL	NKG2 molecule	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel NKG2-specific mAb ( termed P25 ) has been generated that specifically reacts with both NKG2-A and NKG2-C molecules , but fails to recognize NKG2-E molecules .
	manualset3
135278	3	406872	5	NULL	NULL	0	NULL	NKG2-C molecule	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel NKG2-specific mAb ( termed P25 ) has been generated that specifically reacts with both NKG2-A and NKG2-C molecules , but fails to recognize NKG2-E molecules .
	manualset3
135279	4	406872	5	NULL	NULL	0	NULL	NKG2-E molecules	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel NKG2-specific mAb ( termed P25 ) has been generated that specifically reacts with both NKG2-A and NKG2-C molecules , but fails to recognize NKG2-E molecules .
	manualset3
135280	1	406873	5	NULL	NULL	0	NULL	Sex 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex , puberty , and the timing of sleep EEG measured adolescent brain maturation .
	manualset3
135281	2	406873	5	NULL	NULL	0	NULL	puberty 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex , puberty , and the timing of sleep EEG measured adolescent brain maturation .
	manualset3
135282	3	406873	5	NULL	NULL	0	NULL	timing	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex , puberty , and the timing of sleep EEG measured adolescent brain maturation .
	manualset3
135283	4	406873	5	NULL	NULL	0	NULL	sleep 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex , puberty , and the timing of sleep EEG measured adolescent brain maturation .
	manualset3
135284	5	406873	5	NULL	NULL	0	NULL	EEG 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex , puberty , and the timing of sleep EEG measured adolescent brain maturation .
	manualset3
135285	6	406873	5	NULL	NULL	0	NULL	adolescent brain maturation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex , puberty , and the timing of sleep EEG measured adolescent brain maturation .
	manualset3
135286	1	406874	5	NULL	NULL	0	NULL	Sex differences	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex differences in gh mRNA expression during development were also examined by using a full-sib family of C. semilaevis , and the gh mRNA was detected at all of the 12 time points sampled from 10 to 380days-old .
	manualset3
135287	2	406874	5	NULL	NULL	0	NULL	gh mRNA expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex differences in gh mRNA expression during development were also examined by using a full-sib family of C. semilaevis , and the gh mRNA was detected at all of the 12 time points sampled from 10 to 380days-old .
	manualset3
135288	3	406874	5	NULL	NULL	0	NULL	development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex differences in gh mRNA expression during development were also examined by using a full-sib family of C. semilaevis , and the gh mRNA was detected at all of the 12 time points sampled from 10 to 380days-old .
	manualset3
135289	4	406874	5	NULL	NULL	0	NULL	full-sib family	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex differences in gh mRNA expression during development were also examined by using a full-sib family of C. semilaevis , and the gh mRNA was detected at all of the 12 time points sampled from 10 to 380days-old .
	manualset3
135290	5	406874	5	NULL	NULL	0	NULL	C. semilaevis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex differences in gh mRNA expression during development were also examined by using a full-sib family of C. semilaevis , and the gh mRNA was detected at all of the 12 time points sampled from 10 to 380days-old .
	manualset3
135291	6	406874	5	NULL	NULL	0	NULL	gh mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex differences in gh mRNA expression during development were also examined by using a full-sib family of C. semilaevis , and the gh mRNA was detected at all of the 12 time points sampled from 10 to 380days-old .
	manualset3
135292	7	406874	5	NULL	NULL	0	NULL	12 time points 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex differences in gh mRNA expression during development were also examined by using a full-sib family of C. semilaevis , and the gh mRNA was detected at all of the 12 time points sampled from 10 to 380days-old .
	manualset3
135293	8	406874	5	NULL	NULL	0	NULL	10 to 380days-old	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex differences in gh mRNA expression during development were also examined by using a full-sib family of C. semilaevis , and the gh mRNA was detected at all of the 12 time points sampled from 10 to 380days-old .
	manualset3
135294	1	406875	5	NULL	NULL	0	NULL	Sex education	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex education should contain information regarding biological , socio-cultural and spiritual dimensions of sexuality , including cognitive , affective and behavioral domains .
	manualset3
135295	2	406875	5	NULL	NULL	0	NULL	information 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex education should contain information regarding biological , socio-cultural and spiritual dimensions of sexuality , including cognitive , affective and behavioral domains .
	manualset3
135296	3	406875	5	NULL	NULL	0	NULL	biological dimensions 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex education should contain information regarding biological , socio-cultural and spiritual dimensions of sexuality , including cognitive , affective and behavioral domains .
	manualset3
135297	4	406875	5	NULL	NULL	0	NULL	socio-cultural dimensions 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex education should contain information regarding biological , socio-cultural and spiritual dimensions of sexuality , including cognitive , affective and behavioral domains .
	manualset3
135298	5	406875	5	NULL	NULL	0	NULL	spiritual dimensions	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex education should contain information regarding biological , socio-cultural and spiritual dimensions of sexuality , including cognitive , affective and behavioral domains .
	manualset3
135299	6	406875	5	NULL	NULL	0	NULL	sexuality 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex education should contain information regarding biological , socio-cultural and spiritual dimensions of sexuality , including cognitive , affective and behavioral domains .
	manualset3
135300	7	406875	5	NULL	NULL	0	NULL	cognitive domain	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex education should contain information regarding biological , socio-cultural and spiritual dimensions of sexuality , including cognitive , affective and behavioral domains .
	manualset3
135301	8	406875	5	NULL	NULL	0	NULL	affective domain	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex education should contain information regarding biological , socio-cultural and spiritual dimensions of sexuality , including cognitive , affective and behavioral domains .
	manualset3
135302	9	406875	5	NULL	NULL	0	NULL	behavioral domain	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex education should contain information regarding biological , socio-cultural and spiritual dimensions of sexuality , including cognitive , affective and behavioral domains .
	manualset3
135303	1	406876	5	NULL	NULL	0	NULL	Sex murder	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex murder and sex aggression .
	manualset3
135304	2	406876	5	NULL	NULL	0	NULL	sex aggression 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex murder and sex aggression .
	manualset3
135305	1	406877	5	NULL	NULL	0	NULL	Sex ratios	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex ratios between species , revealed by the semifield study with decreasing portions of females from control to 1 : 12 to 1 : 2 , were strongly correlated .
	manualset3
135306	2	406877	5	NULL	NULL	0	NULL	species 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex ratios between species , revealed by the semifield study with decreasing portions of females from control to 1 : 12 to 1 : 2 , were strongly correlated .
	manualset3
135307	3	406877	5	NULL	NULL	0	NULL	semifield study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex ratios between species , revealed by the semifield study with decreasing portions of females from control to 1 : 12 to 1 : 2 , were strongly correlated .
	manualset3
135308	4	406877	5	NULL	NULL	0	NULL	decreasing portions	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex ratios between species , revealed by the semifield study with decreasing portions of females from control to 1 : 12 to 1 : 2 , were strongly correlated .
	manualset3
135309	5	406877	5	NULL	NULL	0	NULL	females 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex ratios between species , revealed by the semifield study with decreasing portions of females from control to 1 : 12 to 1 : 2 , were strongly correlated .
	manualset3
135310	6	406877	5	NULL	NULL	0	NULL	control 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex ratios between species , revealed by the semifield study with decreasing portions of females from control to 1 : 12 to 1 : 2 , were strongly correlated .
	manualset3
135311	7	406877	5	NULL	NULL	0	NULL	1 : 12	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex ratios between species , revealed by the semifield study with decreasing portions of females from control to 1 : 12 to 1 : 2 , were strongly correlated .
	manualset3
135312	8	406877	5	NULL	NULL	0	NULL	1 : 2 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sex ratios between species , revealed by the semifield study with decreasing portions of females from control to 1 : 12 to 1 : 2 , were strongly correlated .
	manualset3
135313	1	406878	5	NULL	NULL	0	NULL	Sexual dimorphism 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sexual dimorphism was expressed-males were more sensitive to environmental changes than females , especially in monoculture .
	manualset3
135314	2	406878	5	NULL	NULL	0	NULL	males 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sexual dimorphism was expressed-males were more sensitive to environmental changes than females , especially in monoculture .
	manualset3
135315	3	406878	5	NULL	NULL	0	NULL	environmental changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sexual dimorphism was expressed-males were more sensitive to environmental changes than females , especially in monoculture .
	manualset3
135316	4	406878	5	NULL	NULL	0	NULL	females 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sexual dimorphism was expressed-males were more sensitive to environmental changes than females , especially in monoculture .
	manualset3
135317	5	406878	5	NULL	NULL	0	NULL	monoculture 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sexual dimorphism was expressed-males were more sensitive to environmental changes than females , especially in monoculture .
	manualset3
135318	1	406879	5	NULL	NULL	0	NULL	amperometric ethanol biosensor	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel amperometric ethanol biosensor was constructed using alcohol dehydrogenase ( ADH ) physically immobilized within poly ( vinyl alcohol ) - multiwalled carbon nanotube ( PVA-MWCNT ) composite obtained by a freezing-thawing process .
	manualset3
135319	2	406879	5	NULL	NULL	0	NULL	alcohol dehydrogenase ( ADH )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel amperometric ethanol biosensor was constructed using alcohol dehydrogenase ( ADH ) physically immobilized within poly ( vinyl alcohol ) - multiwalled carbon nanotube ( PVA-MWCNT ) composite obtained by a freezing-thawing process .
	manualset3
135320	3	406879	5	NULL	NULL	0	NULL	poly ( vinyl alcohol ) - multiwalled carbon nanotube ( PVA-MWCNT ) composite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel amperometric ethanol biosensor was constructed using alcohol dehydrogenase ( ADH ) physically immobilized within poly ( vinyl alcohol ) - multiwalled carbon nanotube ( PVA-MWCNT ) composite obtained by a freezing-thawing process .
	manualset3
135321	4	406879	5	NULL	NULL	0	NULL	freezing-thawing process	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel amperometric ethanol biosensor was constructed using alcohol dehydrogenase ( ADH ) physically immobilized within poly ( vinyl alcohol ) - multiwalled carbon nanotube ( PVA-MWCNT ) composite obtained by a freezing-thawing process .
	manualset3
135322	1	406880	5	NULL	NULL	NULL	NULL	Sham cerclage	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Sham cerclage and local scleral buckle did not decrease blood flow .
	manualset3
135323	2	406880	5	NULL	NULL	0	NULL	local scleral buckle	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Sham cerclage and local scleral buckle did not decrease blood flow .
	manualset3
135325	4	406880	5	NULL	NULL	0	NULL	blood flow	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sham cerclage and local scleral buckle did not decrease blood flow .
	manualset3
135326	1	406881	5	NULL	NULL	0	NULL	Shape priming	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Shape priming was studied in four experiments comprising a complex search task in which subjects searched for a target shape presented among three distractors and reported the location of the target .
	manualset3
135327	2	406881	5	NULL	NULL	0	NULL	four 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Shape priming was studied in four experiments comprising a complex search task in which subjects searched for a target shape presented among three distractors and reported the location of the target .
	manualset3
135328	3	406881	5	NULL	NULL	0	NULL	experiments 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Shape priming was studied in four experiments comprising a complex search task in which subjects searched for a target shape presented among three distractors and reported the location of the target .
	manualset3
135329	4	406881	5	NULL	NULL	0	NULL	complex search task 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Shape priming was studied in four experiments comprising a complex search task in which subjects searched for a target shape presented among three distractors and reported the location of the target .
	manualset3
135330	5	406881	5	NULL	NULL	0	NULL	subjects 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Shape priming was studied in four experiments comprising a complex search task in which subjects searched for a target shape presented among three distractors and reported the location of the target .
	manualset3
135331	6	406881	5	NULL	NULL	0	NULL	target shape	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Shape priming was studied in four experiments comprising a complex search task in which subjects searched for a target shape presented among three distractors and reported the location of the target .
	manualset3
135332	7	406881	5	NULL	NULL	0	NULL	three 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Shape priming was studied in four experiments comprising a complex search task in which subjects searched for a target shape presented among three distractors and reported the location of the target .
	manualset3
135333	8	406881	5	NULL	NULL	0	NULL	distractors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Shape priming was studied in four experiments comprising a complex search task in which subjects searched for a target shape presented among three distractors and reported the location of the target .
	manualset3
135334	9	406881	5	NULL	NULL	0	NULL	location 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Shape priming was studied in four experiments comprising a complex search task in which subjects searched for a target shape presented among three distractors and reported the location of the target .
	manualset3
135335	10	406881	5	NULL	NULL	0	NULL	target 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Shape priming was studied in four experiments comprising a complex search task in which subjects searched for a target shape presented among three distractors and reported the location of the target .
	manualset3
135336	1	406882	5	NULL	NULL	0	NULL	Shared ancestry 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Shared ancestry , evolving stories : similar and contrasting life experiences described by foreign born and U.S. born Latino parents .
	manualset3
135337	2	406882	5	NULL	NULL	0	NULL	evolving stories	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Shared ancestry , evolving stories : similar and contrasting life experiences described by foreign born and U.S. born Latino parents .
	manualset3
135338	3	406882	5	NULL	NULL	0	NULL	life experiences 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Shared ancestry , evolving stories : similar and contrasting life experiences described by foreign born and U.S. born Latino parents .
	manualset3
135339	4	406882	5	NULL	NULL	0	NULL	foreign born Latino parents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Shared ancestry , evolving stories : similar and contrasting life experiences described by foreign born and U.S. born Latino parents .
	manualset3
135340	5	406882	5	NULL	NULL	0	NULL	U.S. born Latino parents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Shared ancestry , evolving stories : similar and contrasting life experiences described by foreign born and U.S. born Latino parents .
	manualset3
135341	1	406883	5	NULL	NULL	0	NULL	Shared care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Shared care between general practitioners and urologists in the management of benign prostatic hyperplasia : a survey of attitudes among clinicians .
	manualset3
135342	2	406883	5	NULL	NULL	0	NULL	general practitioners	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Shared care between general practitioners and urologists in the management of benign prostatic hyperplasia : a survey of attitudes among clinicians .
	manualset3
135343	3	406883	5	NULL	NULL	0	NULL	urologists 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Shared care between general practitioners and urologists in the management of benign prostatic hyperplasia : a survey of attitudes among clinicians .
	manualset3
135344	4	406883	5	NULL	NULL	0	NULL	management 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Shared care between general practitioners and urologists in the management of benign prostatic hyperplasia : a survey of attitudes among clinicians .
	manualset3
135345	5	406883	5	NULL	NULL	0	NULL	benign prostatic hyperplasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Shared care between general practitioners and urologists in the management of benign prostatic hyperplasia : a survey of attitudes among clinicians .
	manualset3
135346	6	406883	5	NULL	NULL	0	NULL	survey 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Shared care between general practitioners and urologists in the management of benign prostatic hyperplasia : a survey of attitudes among clinicians .
	manualset3
135347	7	406883	5	NULL	NULL	0	NULL	attitudes 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Shared care between general practitioners and urologists in the management of benign prostatic hyperplasia : a survey of attitudes among clinicians .
	manualset3
135348	8	406883	5	NULL	NULL	0	NULL	clinicians 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Shared care between general practitioners and urologists in the management of benign prostatic hyperplasia : a survey of attitudes among clinicians .
	manualset3
135349	1	406884	5	NULL	NULL	0	NULL	prescription medication	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Sharing prescription medication among teenage girls : potential danger to unplanned/undiagnosed pregnancies .
	manualset3
135350	2	406884	5	NULL	NULL	0	NULL	teenage girls 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sharing prescription medication among teenage girls : potential danger to unplanned/undiagnosed pregnancies .
	manualset3
135351	3	406884	5	NULL	NULL	0	NULL	potential danger 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sharing prescription medication among teenage girls : potential danger to unplanned/undiagnosed pregnancies .
	manualset3
135352	4	406884	5	NULL	NULL	0	NULL	unplanned/undiagnosed pregnancies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sharing prescription medication among teenage girls : potential danger to unplanned/undiagnosed pregnancies .
	manualset3
135353	1	406885	5	NULL	NULL	0	NULL	atopy requiring treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	She also had atopy requiring treatment to control asthma and eczema .
	manualset3
135355	3	406885	5	NULL	NULL	0	NULL	asthma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	She also had atopy requiring treatment to control asthma and eczema .
	manualset3
135356	4	406885	5	NULL	NULL	0	NULL	eczema 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	She also had atopy requiring treatment to control asthma and eczema .
	manualset3
135357	1	406886	5	NULL	NULL	0	NULL	Catechin dimers 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	( Catechin dimers of oak bark .
	manualset3
135358	2	406886	5	NULL	NULL	0	NULL	oak bark 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Catechin dimers of oak bark .
	manualset3
135359	1	406887	5	NULL	NULL	0	NULL	 cloud point extraction procedure 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel and sensitive cloud point extraction procedure for the determination of trace amounts of malachite green by spectrophotometry was developed .
	manualset3
135360	2	406887	5	NULL	NULL	0	NULL	determination 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel and sensitive cloud point extraction procedure for the determination of trace amounts of malachite green by spectrophotometry was developed .
	manualset3
135361	3	406887	5	NULL	NULL	0	NULL	trace amounts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel and sensitive cloud point extraction procedure for the determination of trace amounts of malachite green by spectrophotometry was developed .
	manualset3
135362	4	406887	5	NULL	NULL	0	NULL	malachite green	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel and sensitive cloud point extraction procedure for the determination of trace amounts of malachite green by spectrophotometry was developed .
	manualset3
135363	5	406887	5	NULL	NULL	0	NULL	spectrophotometry 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel and sensitive cloud point extraction procedure for the determination of trace amounts of malachite green by spectrophotometry was developed .
	manualset3
135364	1	406888	5	NULL	NULL	0	NULL	pregnant 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	She became pregnant following intra-tubal insemination and the value and limitations of such a procedure are discussed .
	manualset3
135365	2	406888	5	NULL	NULL	0	NULL	intra-tubal insemination 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	She became pregnant following intra-tubal insemination and the value and limitations of such a procedure are discussed .
	manualset3
135366	3	406888	5	NULL	NULL	0	NULL	value 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	She became pregnant following intra-tubal insemination and the value and limitations of such a procedure are discussed .
	manualset3
135367	4	406888	5	NULL	NULL	0	NULL	limitations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	She became pregnant following intra-tubal insemination and the value and limitations of such a procedure are discussed .
	manualset3
135368	5	406888	5	NULL	NULL	0	NULL	procedure 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	She became pregnant following intra-tubal insemination and the value and limitations of such a procedure are discussed .
	manualset3
135369	1	406889	5	NULL	NULL	NULL	NULL	cone-shaped calvarium	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	She had a cone-shaped calvarium , midface hypoplasia , syndactyly of the hands and feet , hypertelorism , proptosis and cleft palate .
	manualset3
135370	2	406889	5	NULL	NULL	0	NULL	midface hypoplasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	She had a cone-shaped calvarium , midface hypoplasia , syndactyly of the hands and feet , hypertelorism , proptosis and cleft palate .
	manualset3
135371	3	406889	5	NULL	NULL	0	NULL	syndactyly 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	She had a cone-shaped calvarium , midface hypoplasia , syndactyly of the hands and feet , hypertelorism , proptosis and cleft palate .
	manualset3
135372	4	406889	5	NULL	NULL	0	NULL	hands 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	She had a cone-shaped calvarium , midface hypoplasia , syndactyly of the hands and feet , hypertelorism , proptosis and cleft palate .
	manualset3
135373	5	406889	5	NULL	NULL	0	NULL	feet 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	She had a cone-shaped calvarium , midface hypoplasia , syndactyly of the hands and feet , hypertelorism , proptosis and cleft palate .
	manualset3
135374	6	406889	5	NULL	NULL	0	NULL	hypertelorism 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	She had a cone-shaped calvarium , midface hypoplasia , syndactyly of the hands and feet , hypertelorism , proptosis and cleft palate .
	manualset3
135375	7	406889	5	NULL	NULL	0	NULL	proptosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	She had a cone-shaped calvarium , midface hypoplasia , syndactyly of the hands and feet , hypertelorism , proptosis and cleft palate .
	manualset3
135376	8	406889	5	NULL	NULL	0	NULL	cleft palate 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	She had a cone-shaped calvarium , midface hypoplasia , syndactyly of the hands and feet , hypertelorism , proptosis and cleft palate .
	manualset3
135377	1	406890	5	NULL	NULL	0	NULL	low concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	She had a low concentration of plasma protein C on admission to hospital and during the follow up .
	manualset3
135378	2	406890	5	NULL	NULL	0	NULL	plasma protein C	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	She had a low concentration of plasma protein C on admission to hospital and during the follow up .
	manualset3
135379	3	406890	5	NULL	NULL	0	NULL	admission 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	She had a low concentration of plasma protein C on admission to hospital and during the follow up .
	manualset3
135380	4	406890	5	NULL	NULL	0	NULL	hospital 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	She had a low concentration of plasma protein C on admission to hospital and during the follow up .
	manualset3
135381	5	406890	5	NULL	NULL	NULL	NULL	follow up	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	She had a low concentration of plasma protein C on admission to hospital and during the follow up .
	manualset3
135382	1	406891	5	NULL	NULL	0	NULL	past history	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	She had a past history of hypersensitivity to mosquito bites ( HMB ) .
	manualset3
135383	2	406891	5	NULL	NULL	NULL	NULL	hypersensitivity to mosquito bites ( HMB )	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	She had a past history of hypersensitivity to mosquito bites ( HMB ) .
	manualset3
135384	1	406892	5	NULL	NULL	0	NULL	symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	She had hed these symptomes for six months prior to admission , but denied lifelong bleeding tendency .
	manualset3
135385	2	406892	5	NULL	NULL	0	NULL	six months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	She had hed these symptomes for six months prior to admission , but denied lifelong bleeding tendency .
	manualset3
135386	3	406892	5	NULL	NULL	0	NULL	admission 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	She had hed these symptomes for six months prior to admission , but denied lifelong bleeding tendency .
	manualset3
135387	4	406892	5	NULL	NULL	0	NULL	lifelong bleeding tendency 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	She had hed these symptomes for six months prior to admission , but denied lifelong bleeding tendency .
	manualset3
135388	1	406893	5	NULL	NULL	0	NULL	skeletal Class II malocclusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	She presented clinically with a skeletal Class II malocclusion with severe overbite and overjet .
	manualset3
135389	2	406893	5	NULL	NULL	0	NULL	overbite 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	She presented clinically with a skeletal Class II malocclusion with severe overbite and overjet .
	manualset3
135390	3	406893	5	NULL	NULL	0	NULL	overjet 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	She presented clinically with a skeletal Class II malocclusion with severe overbite and overjet .
	manualset3
135391	1	406894	5	NULL	NULL	0	NULL	wide excision	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	She underwent wide excision of the lesions that revealed metastasis of TCC .
	manualset3
135392	2	406894	5	NULL	NULL	0	NULL	lesions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	She underwent wide excision of the lesions that revealed metastasis of TCC .
	manualset3
135393	3	406894	5	NULL	NULL	0	NULL	metastasis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	She underwent wide excision of the lesions that revealed metastasis of TCC .
	manualset3
135394	4	406894	5	NULL	NULL	0	NULL	TCC 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	She underwent wide excision of the lesions that revealed metastasis of TCC .
	manualset3
135395	1	406895	5	NULL	NULL	0	NULL	pneumonia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	She was diagnosed to have pneumonia based on the clinical , radiological and laboratory findings , and empirical antibiotic treatment with ciprofloxacin and ceftazidime combination was initiated .
	manualset3
135396	2	406895	5	NULL	NULL	0	NULL	clinical findings 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	She was diagnosed to have pneumonia based on the clinical , radiological and laboratory findings , and empirical antibiotic treatment with ciprofloxacin and ceftazidime combination was initiated .
	manualset3
135397	3	406895	5	NULL	NULL	0	NULL	radiological findings 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	She was diagnosed to have pneumonia based on the clinical , radiological and laboratory findings , and empirical antibiotic treatment with ciprofloxacin and ceftazidime combination was initiated .
	manualset3
135398	4	406895	5	NULL	NULL	0	NULL	laboratory findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	She was diagnosed to have pneumonia based on the clinical , radiological and laboratory findings , and empirical antibiotic treatment with ciprofloxacin and ceftazidime combination was initiated .
	manualset3
135399	5	406895	5	NULL	NULL	0	NULL	empirical antibiotic treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	She was diagnosed to have pneumonia based on the clinical , radiological and laboratory findings , and empirical antibiotic treatment with ciprofloxacin and ceftazidime combination was initiated .
	manualset3
135400	6	406895	5	NULL	NULL	0	NULL	ciprofloxacin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	She was diagnosed to have pneumonia based on the clinical , radiological and laboratory findings , and empirical antibiotic treatment with ciprofloxacin and ceftazidime combination was initiated .
	manualset3
135401	7	406895	5	NULL	NULL	0	NULL	ceftazidime 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	She was diagnosed to have pneumonia based on the clinical , radiological and laboratory findings , and empirical antibiotic treatment with ciprofloxacin and ceftazidime combination was initiated .
	manualset3
135402	1	406896	5	NULL	NULL	0	NULL	cardiac tamponade	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	She was found to have cardiac tamponade and pneumothorax .
	manualset3
135403	2	406896	5	NULL	NULL	0	NULL	pneumothorax 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	She was found to have cardiac tamponade and pneumothorax .
	manualset3
135404	1	406897	5	NULL	NULL	0	NULL	gluten-free diet 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	She was on a gluten-free diet because of a celiac disease which had been diagnosed 3 months before .
	manualset3
135405	2	406897	5	NULL	NULL	0	NULL	celiac disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	She was on a gluten-free diet because of a celiac disease which had been diagnosed 3 months before .
	manualset3
135406	3	406897	5	NULL	NULL	0	NULL	3 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	She was on a gluten-free diet because of a celiac disease which had been diagnosed 3 months before .
	manualset3
135407	1	406898	5	NULL	NULL	0	NULL	breast abscess	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	She was treated surgically as breast abscess which failed to resolve in due course .
	manualset3
135408	2	406898	5	NULL	NULL	0	NULL	due course	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	She was treated surgically as breast abscess which failed to resolve in due course .
	manualset3
135409	1	406899	5	NULL	NULL	0	NULL	Sheep red cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Sheep red cells , sensitized with a genus-specific leptospiral substance extracted from a water leptospira , were preserved by freeze drying .
	manualset3
135410	2	406899	5	NULL	NULL	0	NULL	genus-specific leptospiral substance	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sheep red cells , sensitized with a genus-specific leptospiral substance extracted from a water leptospira , were preserved by freeze drying .
	manualset3
135411	3	406899	5	NULL	NULL	0	NULL	water leptospira 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sheep red cells , sensitized with a genus-specific leptospiral substance extracted from a water leptospira , were preserved by freeze drying .
	manualset3
135412	4	406899	5	NULL	NULL	0	NULL	freeze drying	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sheep red cells , sensitized with a genus-specific leptospiral substance extracted from a water leptospira , were preserved by freeze drying .
	manualset3
135413	1	406900	5	NULL	NULL	0	NULL	Shewanellae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Shewanellae are microbial models for environmental stress response ; however , the sequential expression of mechanisms in response to stress is poorly understood .
	manualset3
135414	2	406900	5	NULL	NULL	0	NULL	microbial models	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Shewanellae are microbial models for environmental stress response ; however , the sequential expression of mechanisms in response to stress is poorly understood .
	manualset3
135415	3	406900	5	NULL	NULL	0	NULL	environmental stress response 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Shewanellae are microbial models for environmental stress response ; however , the sequential expression of mechanisms in response to stress is poorly understood .
	manualset3
135416	4	406900	5	NULL	NULL	0	NULL	sequential expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Shewanellae are microbial models for environmental stress response ; however , the sequential expression of mechanisms in response to stress is poorly understood .
	manualset3
135417	5	406900	5	NULL	NULL	0	NULL	mechanisms 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Shewanellae are microbial models for environmental stress response ; however , the sequential expression of mechanisms in response to stress is poorly understood .
	manualset3
135418	6	406900	5	NULL	NULL	0	NULL	response 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Shewanellae are microbial models for environmental stress response ; however , the sequential expression of mechanisms in response to stress is poorly understood .
	manualset3
135419	7	406900	5	NULL	NULL	0	NULL	stress 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Shewanellae are microbial models for environmental stress response ; however , the sequential expression of mechanisms in response to stress is poorly understood .
	manualset3
135420	1	406901	5	NULL	NULL	0	NULL	Short-circuit currents	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Short-circuit currents through tissue were monitored for changes that might have been observed under ion-cyclotron resonance ( ICR ) conditions for each of several ions : H + , Li + , Na + , K + , Ca2 + , and Cl - .
	manualset3
135421	2	406901	5	NULL	NULL	0	NULL	tissue 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Short-circuit currents through tissue were monitored for changes that might have been observed under ion-cyclotron resonance ( ICR ) conditions for each of several ions : H + , Li + , Na + , K + , Ca2 + , and Cl - .
	manualset3
135422	3	406901	5	NULL	NULL	0	NULL	changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Short-circuit currents through tissue were monitored for changes that might have been observed under ion-cyclotron resonance ( ICR ) conditions for each of several ions : H + , Li + , Na + , K + , Ca2 + , and Cl - .
	manualset3
135423	4	406901	5	NULL	NULL	0	NULL	ion-cyclotron resonance ( ICR ) conditions  	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Short-circuit currents through tissue were monitored for changes that might have been observed under ion-cyclotron resonance ( ICR ) conditions for each of several ions : H + , Li + , Na + , K + , Ca2 + , and Cl - .
	manualset3
135424	5	406901	5	NULL	NULL	0	NULL	ions 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Short-circuit currents through tissue were monitored for changes that might have been observed under ion-cyclotron resonance ( ICR ) conditions for each of several ions : H + , Li + , Na + , K + , Ca2 + , and Cl - .
	manualset3
135425	6	406901	5	NULL	NULL	0	NULL	H +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Short-circuit currents through tissue were monitored for changes that might have been observed under ion-cyclotron resonance ( ICR ) conditions for each of several ions : H + , Li + , Na + , K + , Ca2 + , and Cl - .
	manualset3
135426	7	406901	5	NULL	NULL	0	NULL	Li +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Short-circuit currents through tissue were monitored for changes that might have been observed under ion-cyclotron resonance ( ICR ) conditions for each of several ions : H + , Li + , Na + , K + , Ca2 + , and Cl - .
	manualset3
135427	8	406901	5	NULL	NULL	0	NULL	Na +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Short-circuit currents through tissue were monitored for changes that might have been observed under ion-cyclotron resonance ( ICR ) conditions for each of several ions : H + , Li + , Na + , K + , Ca2 + , and Cl - .
	manualset3
135428	9	406901	5	NULL	NULL	0	NULL	K +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Short-circuit currents through tissue were monitored for changes that might have been observed under ion-cyclotron resonance ( ICR ) conditions for each of several ions : H + , Li + , Na + , K + , Ca2 + , and Cl - .
	manualset3
135429	10	406901	5	NULL	NULL	0	NULL	Ca2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Short-circuit currents through tissue were monitored for changes that might have been observed under ion-cyclotron resonance ( ICR ) conditions for each of several ions : H + , Li + , Na + , K + , Ca2 + , and Cl - .
	manualset3
135430	11	406901	5	NULL	NULL	0	NULL	Cl -	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Short-circuit currents through tissue were monitored for changes that might have been observed under ion-cyclotron resonance ( ICR ) conditions for each of several ions : H + , Li + , Na + , K + , Ca2 + , and Cl - .
	manualset3
135431	1	406902	5	NULL	NULL	NULL	NULL	Short-lived carriage 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Short-lived carriage of foot-and-mouth disease virus in human nasal cavities after exposure to infected animals .
	manualset3
135432	2	406902	5	NULL	NULL	0	NULL	foot-and-mouth disease virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Short-lived carriage of foot-and-mouth disease virus in human nasal cavities after exposure to infected animals .
	manualset3
135433	3	406902	5	NULL	NULL	0	NULL	human nasal cavities 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Short-lived carriage of foot-and-mouth disease virus in human nasal cavities after exposure to infected animals .
	manualset3
135434	4	406902	5	NULL	NULL	0	NULL	exposure 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Short-lived carriage of foot-and-mouth disease virus in human nasal cavities after exposure to infected animals .
	manualset3
135435	5	406902	5	NULL	NULL	0	NULL	infected animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Short-lived carriage of foot-and-mouth disease virus in human nasal cavities after exposure to infected animals .
	manualset3
135436	1	406903	5	NULL	NULL	0	NULL	Short-path statistics	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Short-path statistics and the diffusion approximation .
	manualset3
135437	2	406903	5	NULL	NULL	0	NULL	diffusion approximation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Short-path statistics and the diffusion approximation .
	manualset3
135438	1	406904	5	NULL	NULL	NULL	NULL	Short-term effects	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Short-term effects were examined 2 hours after consumption of 450 mL tea or water .
	manualset3
135439	2	406904	5	NULL	NULL	0	NULL	2 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Short-term effects were examined 2 hours after consumption of 450 mL tea or water .
	manualset3
135440	3	406904	5	NULL	NULL	0	NULL	consumption 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Short-term effects were examined 2 hours after consumption of 450 mL tea or water .
	manualset3
135441	4	406904	5	NULL	NULL	0	NULL	450 mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Short-term effects were examined 2 hours after consumption of 450 mL tea or water .
	manualset3
135442	5	406904	5	NULL	NULL	0	NULL	tea 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Short-term effects were examined 2 hours after consumption of 450 mL tea or water .
	manualset3
135443	6	406904	5	NULL	NULL	0	NULL	water 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Short-term effects were examined 2 hours after consumption of 450 mL tea or water .
	manualset3
135444	1	406905	5	NULL	NULL	0	NULL	 novel approach 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel approach for the description of the protein stoichiometry of viral capsids , that is the protein shells protecting the viral genome , is introduced based on tiling theory .
	manualset3
135445	2	406905	5	NULL	NULL	0	NULL	description 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel approach for the description of the protein stoichiometry of viral capsids , that is the protein shells protecting the viral genome , is introduced based on tiling theory .
	manualset3
135446	3	406905	5	NULL	NULL	0	NULL	protein stoichiometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel approach for the description of the protein stoichiometry of viral capsids , that is the protein shells protecting the viral genome , is introduced based on tiling theory .
	manualset3
135447	4	406905	5	NULL	NULL	0	NULL	viral capsids	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel approach for the description of the protein stoichiometry of viral capsids , that is the protein shells protecting the viral genome , is introduced based on tiling theory .
	manualset3
135448	5	406905	5	NULL	NULL	0	NULL	protein shells 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel approach for the description of the protein stoichiometry of viral capsids , that is the protein shells protecting the viral genome , is introduced based on tiling theory .
	manualset3
135449	6	406905	5	NULL	NULL	0	NULL	viral genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel approach for the description of the protein stoichiometry of viral capsids , that is the protein shells protecting the viral genome , is introduced based on tiling theory .
	manualset3
135450	7	406905	5	NULL	NULL	0	NULL	tiling theory	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel approach for the description of the protein stoichiometry of viral capsids , that is the protein shells protecting the viral genome , is introduced based on tiling theory .
	manualset3
135451	1	406906	5	NULL	NULL	0	NULL	Short-term precision	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Short-term precision in vivo was expressed as root mean square standard deviation of paired measurements of 20 healthy volunteers ( RMSSD = 0.5 % ) .
	manualset3
135452	2	406906	5	NULL	NULL	0	NULL	root mean square standard deviation	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Short-term precision in vivo was expressed as root mean square standard deviation of paired measurements of 20 healthy volunteers ( RMSSD = 0.5 % ) .
	manualset3
135453	3	406906	5	NULL	NULL	0	NULL	paired measurements	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Short-term precision in vivo was expressed as root mean square standard deviation of paired measurements of 20 healthy volunteers ( RMSSD = 0.5 % ) .
	manualset3
135454	4	406906	5	NULL	NULL	0	NULL	20 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Short-term precision in vivo was expressed as root mean square standard deviation of paired measurements of 20 healthy volunteers ( RMSSD = 0.5 % ) .
	manualset3
135455	5	406906	5	NULL	NULL	0	NULL	healthy volunteers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Short-term precision in vivo was expressed as root mean square standard deviation of paired measurements of 20 healthy volunteers ( RMSSD = 0.5 % ) .
	manualset3
135456	6	406906	5	NULL	NULL	0	NULL	RMSSD = 0.5 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Short-term precision in vivo was expressed as root mean square standard deviation of paired measurements of 20 healthy volunteers ( RMSSD = 0.5 % ) .
	manualset3
135457	1	406907	5	NULL	NULL	0	NULL	Short C-HO hydrogen-bonding inter-actions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Short C-HO hydrogen-bonding inter-actions between meth-oxy groups result in a one-dimensional polymeric chain of mol-ecules lying parallel to the b axis .
	manualset3
135458	2	406907	5	NULL	NULL	0	NULL	meth-oxy groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Short C-HO hydrogen-bonding inter-actions between meth-oxy groups result in a one-dimensional polymeric chain of mol-ecules lying parallel to the b axis .
	manualset3
135459	3	406907	5	NULL	NULL	0	NULL	one-dimensional polymeric chain	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Short C-HO hydrogen-bonding inter-actions between meth-oxy groups result in a one-dimensional polymeric chain of mol-ecules lying parallel to the b axis .
	manualset3
135460	4	406907	5	NULL	NULL	0	NULL	mol-ecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Short C-HO hydrogen-bonding inter-actions between meth-oxy groups result in a one-dimensional polymeric chain of mol-ecules lying parallel to the b axis .
	manualset3
135461	5	406907	5	NULL	NULL	0	NULL	b axis	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Short C-HO hydrogen-bonding inter-actions between meth-oxy groups result in a one-dimensional polymeric chain of mol-ecules lying parallel to the b axis .
	manualset3
135462	1	406908	5	NULL	NULL	0	NULL	Short birth intervals	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Short birth intervals also have negative effects on the offspring .
	manualset3
135463	2	406908	5	NULL	NULL	0	NULL	negative effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Short birth intervals also have negative effects on the offspring .
	manualset3
135464	3	406908	5	NULL	NULL	0	NULL	offspring 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Short birth intervals also have negative effects on the offspring .
	manualset3
135465	1	406909	5	NULL	NULL	0	NULL	Short cultural life span	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Short cultural life span , regular growth and positive secretion activity are typical of low-grade tumors , meanwhile the opposite is true for high-grade tumors .
	manualset3
135466	2	406909	5	NULL	NULL	0	NULL	regular growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Short cultural life span , regular growth and positive secretion activity are typical of low-grade tumors , meanwhile the opposite is true for high-grade tumors .
	manualset3
135467	3	406909	5	NULL	NULL	0	NULL	positive secretion activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Short cultural life span , regular growth and positive secretion activity are typical of low-grade tumors , meanwhile the opposite is true for high-grade tumors .
	manualset3
135468	4	406909	5	NULL	NULL	0	NULL	low-grade tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Short cultural life span , regular growth and positive secretion activity are typical of low-grade tumors , meanwhile the opposite is true for high-grade tumors .
	manualset3
135469	5	406909	5	NULL	NULL	0	NULL	 high-grade tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Short cultural life span , regular growth and positive secretion activity are typical of low-grade tumors , meanwhile the opposite is true for high-grade tumors .
	manualset3
135470	1	406910	5	NULL	NULL	0	NULL	Short report 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Short report : evidence of worldwide transmission of hepatitis G virus .
	manualset3
135471	2	406910	5	NULL	NULL	0	NULL	evidence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Short report : evidence of worldwide transmission of hepatitis G virus .
	manualset3
135472	3	406910	5	NULL	NULL	0	NULL	worldwide transmission	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Short report : evidence of worldwide transmission of hepatitis G virus .
	manualset3
135473	4	406910	5	NULL	NULL	0	NULL	hepatitis G virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Short report : evidence of worldwide transmission of hepatitis G virus .
	manualset3
135474	1	406911	5	NULL	NULL	0	NULL	intravenous immunization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Shortly after intravenous immunization of mice with heterologous erythrocytes ( RBC ) antigen-specific Thy 1 + cells which form rosettes with the immunizing RBC ( thymic-derived lymphocytes-forming rosettes ( T-RFC ) ) appear in the spleen .
	manualset3
135475	2	406911	5	NULL	NULL	0	NULL	mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Shortly after intravenous immunization of mice with heterologous erythrocytes ( RBC ) antigen-specific Thy 1 + cells which form rosettes with the immunizing RBC ( thymic-derived lymphocytes-forming rosettes ( T-RFC ) ) appear in the spleen .
	manualset3
135476	3	406911	5	NULL	NULL	0	NULL	heterologous erythrocytes ( RBC ) antigen-specific Thy 1 + cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Shortly after intravenous immunization of mice with heterologous erythrocytes ( RBC ) antigen-specific Thy 1 + cells which form rosettes with the immunizing RBC ( thymic-derived lymphocytes-forming rosettes ( T-RFC ) ) appear in the spleen .
	manualset3
135477	4	406911	5	NULL	NULL	0	NULL	rosettes 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Shortly after intravenous immunization of mice with heterologous erythrocytes ( RBC ) antigen-specific Thy 1 + cells which form rosettes with the immunizing RBC ( thymic-derived lymphocytes-forming rosettes ( T-RFC ) ) appear in the spleen .
	manualset3
135478	5	406911	5	NULL	NULL	0	NULL	RBC 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Shortly after intravenous immunization of mice with heterologous erythrocytes ( RBC ) antigen-specific Thy 1 + cells which form rosettes with the immunizing RBC ( thymic-derived lymphocytes-forming rosettes ( T-RFC ) ) appear in the spleen .
	manualset3
135479	6	406911	5	NULL	NULL	0	NULL	thymic-derived lymphocytes-forming rosettes ( T-RFC )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Shortly after intravenous immunization of mice with heterologous erythrocytes ( RBC ) antigen-specific Thy 1 + cells which form rosettes with the immunizing RBC ( thymic-derived lymphocytes-forming rosettes ( T-RFC ) ) appear in the spleen .
	manualset3
135480	7	406911	5	NULL	NULL	0	NULL	spleen 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Shortly after intravenous immunization of mice with heterologous erythrocytes ( RBC ) antigen-specific Thy 1 + cells which form rosettes with the immunizing RBC ( thymic-derived lymphocytes-forming rosettes ( T-RFC ) ) appear in the spleen .
	manualset3
135481	1	406912	5	NULL	NULL	0	NULL	approach 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel approach to visualize biological sequences is developed based on cellular automata ( Wolfram , S. Nature 1984 , 311 , 419-424 ) , a set of discrete dynamical systems in which space and time are discrete .
	manualset3
135482	2	406912	5	NULL	NULL	0	NULL	biological sequences	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel approach to visualize biological sequences is developed based on cellular automata ( Wolfram , S. Nature 1984 , 311 , 419-424 ) , a set of discrete dynamical systems in which space and time are discrete .
	manualset3
135483	3	406912	5	NULL	NULL	NULL	NULL	cellular automata	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A novel approach to visualize biological sequences is developed based on cellular automata ( Wolfram , S. Nature 1984 , 311 , 419-424 ) , a set of discrete dynamical systems in which space and time are discrete .
	manualset3
135484	4	406912	5	NULL	NULL	0	NULL	Wolfram , S. Nature 1984 , 311 , 419-424 	Citation												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel approach to visualize biological sequences is developed based on cellular automata ( Wolfram , S. Nature 1984 , 311 , 419-424 ) , a set of discrete dynamical systems in which space and time are discrete .
	manualset3
135485	5	406912	5	NULL	NULL	0	NULL	set of discrete dynamical systems	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel approach to visualize biological sequences is developed based on cellular automata ( Wolfram , S. Nature 1984 , 311 , 419-424 ) , a set of discrete dynamical systems in which space and time are discrete .
	manualset3
135486	6	406912	5	NULL	NULL	0	NULL	space 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel approach to visualize biological sequences is developed based on cellular automata ( Wolfram , S. Nature 1984 , 311 , 419-424 ) , a set of discrete dynamical systems in which space and time are discrete .
	manualset3
135487	7	406912	5	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel approach to visualize biological sequences is developed based on cellular automata ( Wolfram , S. Nature 1984 , 311 , 419-424 ) , a set of discrete dynamical systems in which space and time are discrete .
	manualset3
135488	1	406913	5	NULL	NULL	0	NULL	OHT 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Should OHT compete with CT to stage the mediastinum noninvasively in lung cancer ?
	manualset3
135489	2	406913	5	NULL	NULL	0	NULL	CT 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Should OHT compete with CT to stage the mediastinum noninvasively in lung cancer ?
	manualset3
135490	3	406913	5	NULL	NULL	0	NULL	mediastinum 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Should OHT compete with CT to stage the mediastinum noninvasively in lung cancer ?
	manualset3
135491	4	406913	5	NULL	NULL	0	NULL	lung cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Should OHT compete with CT to stage the mediastinum noninvasively in lung cancer ?
	manualset3
135492	1	406914	5	NULL	NULL	0	NULL	hepatitits-C virus antibody-positive donors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Should hepatitits-C virus antibody-positive donors be excluded from kidney donation ?
	manualset3
135493	2	406914	5	NULL	NULL	0	NULL	kidney donation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Should hepatitits-C virus antibody-positive donors be excluded from kidney donation ?
	manualset3
135494	1	406915	5	NULL	NULL	0	NULL	stroke patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Should all stroke patients receive tissue plasminogen activator therapy , despite mild or improving symptoms ?
	manualset3
135495	2	406915	5	NULL	NULL	0	NULL	tissue plasminogen activator therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Should all stroke patients receive tissue plasminogen activator therapy , despite mild or improving symptoms ?
	manualset3
135496	3	406915	5	NULL	NULL	0	NULL	mild or improving symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Should all stroke patients receive tissue plasminogen activator therapy , despite mild or improving symptoms ?
	manualset3
135497	1	406916	5	NULL	NULL	0	NULL	Shoulder ultrasonography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Shoulder ultrasonography is useful in the diagnosis of full thickness tears , but its utility for other rotator cuff disorders , shoulder impingement syndrome and subacromial bursitis is less well established .
	manualset3
135498	2	406916	5	NULL	NULL	0	NULL	diagnosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Shoulder ultrasonography is useful in the diagnosis of full thickness tears , but its utility for other rotator cuff disorders , shoulder impingement syndrome and subacromial bursitis is less well established .
	manualset3
135499	3	406916	5	NULL	NULL	0	NULL	full thickness tears 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Shoulder ultrasonography is useful in the diagnosis of full thickness tears , but its utility for other rotator cuff disorders , shoulder impingement syndrome and subacromial bursitis is less well established .
	manualset3
135500	4	406916	5	NULL	NULL	0	NULL	utility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Shoulder ultrasonography is useful in the diagnosis of full thickness tears , but its utility for other rotator cuff disorders , shoulder impingement syndrome and subacromial bursitis is less well established .
	manualset3
135501	5	406916	5	NULL	NULL	0	NULL	rotator cuff disorders 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Shoulder ultrasonography is useful in the diagnosis of full thickness tears , but its utility for other rotator cuff disorders , shoulder impingement syndrome and subacromial bursitis is less well established .
	manualset3
135502	6	406916	5	NULL	NULL	0	NULL	shoulder impingement syndrome 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Shoulder ultrasonography is useful in the diagnosis of full thickness tears , but its utility for other rotator cuff disorders , shoulder impingement syndrome and subacromial bursitis is less well established .
	manualset3
135503	7	406916	5	NULL	NULL	0	NULL	subacromial bursitis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Shoulder ultrasonography is useful in the diagnosis of full thickness tears , but its utility for other rotator cuff disorders , shoulder impingement syndrome and subacromial bursitis is less well established .
	manualset3
135504	1	406917	5	NULL	NULL	0	NULL	Shrimp farm activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Shrimp farm activity can elevate in-situ soil salinity that in turn may affect any subsequent crop production if land usage changes .
	manualset3
135505	2	406917	5	NULL	NULL	0	NULL	in-situ soil salinity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Shrimp farm activity can elevate in-situ soil salinity that in turn may affect any subsequent crop production if land usage changes .
	manualset3
135507	4	406917	5	NULL	NULL	0	NULL	crop production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Shrimp farm activity can elevate in-situ soil salinity that in turn may affect any subsequent crop production if land usage changes .
	manualset3
135508	5	406917	5	NULL	NULL	0	NULL	land usage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Shrimp farm activity can elevate in-situ soil salinity that in turn may affect any subsequent crop production if land usage changes .
	manualset3
135509	1	406918	5	NULL	NULL	0	NULL	oxygen 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Shunting of inspired oxygen , presumably due to arteriovenous anastomoses , from tumor feeding arterioles to adjacent venules was imaged .
	manualset3
135510	2	406918	5	NULL	NULL	0	NULL	arteriovenous anastomoses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Shunting of inspired oxygen , presumably due to arteriovenous anastomoses , from tumor feeding arterioles to adjacent venules was imaged .
	manualset3
135511	3	406918	5	NULL	NULL	0	NULL	tumor feeding arterioles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Shunting of inspired oxygen , presumably due to arteriovenous anastomoses , from tumor feeding arterioles to adjacent venules was imaged .
	manualset3
135512	4	406918	5	NULL	NULL	0	NULL	venules 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Shunting of inspired oxygen , presumably due to arteriovenous anastomoses , from tumor feeding arterioles to adjacent venules was imaged .
	manualset3
135513	1	406919	5	NULL	NULL	0	NULL	Sialic acid-dependent recognition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sialic acid-dependent recognition of laminin by Penicillium marneffei conidia .
	manualset3
135514	2	406919	5	NULL	NULL	0	NULL	laminin 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sialic acid-dependent recognition of laminin by Penicillium marneffei conidia .
	manualset3
135515	3	406919	5	NULL	NULL	0	NULL	Penicillium marneffei conidia	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sialic acid-dependent recognition of laminin by Penicillium marneffei conidia .
	manualset3
135516	1	406920	5	NULL	NULL	0	NULL	novel assay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel assay of glucuronidation of C - and N-hydroxylated metabolites of the carcinogen N-2-fluorenylacetamide .
	manualset3
135517	2	406920	5	NULL	NULL	0	NULL	glucuronidation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel assay of glucuronidation of C - and N-hydroxylated metabolites of the carcinogen N-2-fluorenylacetamide .
	manualset3
135518	3	406920	5	NULL	NULL	0	NULL	C -hydroxylated metabolites	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel assay of glucuronidation of C - and N-hydroxylated metabolites of the carcinogen N-2-fluorenylacetamide .
	manualset3
135519	4	406920	5	NULL	NULL	0	NULL	N-hydroxylated metabolites	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel assay of glucuronidation of C - and N-hydroxylated metabolites of the carcinogen N-2-fluorenylacetamide .
	manualset3
135520	5	406920	5	NULL	NULL	0	NULL	carcinogen N-2-fluorenylacetamide 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel assay of glucuronidation of C - and N-hydroxylated metabolites of the carcinogen N-2-fluorenylacetamide .
	manualset3
135521	1	406921	5	NULL	NULL	0	NULL	Sickle cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Sickle cells incorporate less of their 32P into spectrin band 2 and more into band 4.5 than do normal cells .
	manualset3
135522	2	406921	5	NULL	NULL	0	NULL	32P	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Sickle cells incorporate less of their 32P into spectrin band 2 and more into band 4.5 than do normal cells .
	manualset3
135523	3	406921	5	NULL	NULL	NULL	NULL	spectrin band 2	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Sickle cells incorporate less of their 32P into spectrin band 2 and more into band 4.5 than do normal cells .
	manualset3
135524	4	406921	5	NULL	NULL	0	NULL	band 4.5	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sickle cells incorporate less of their 32P into spectrin band 2 and more into band 4.5 than do normal cells .
	manualset3
135525	5	406921	5	NULL	NULL	0	NULL	normal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Sickle cells incorporate less of their 32P into spectrin band 2 and more into band 4.5 than do normal cells .
	manualset3
135526	1	406922	5	NULL	NULL	0	NULL	Side effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Side effects were more common with disopyramide .
	manualset3
135527	2	406922	5	NULL	NULL	0	NULL	disopyramide 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Side effects were more common with disopyramide .
	manualset3
135528	1	406923	5	NULL	NULL	0	NULL	Sieving coefficients	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sieving coefficients of different solutes ranged from 0.1 to 1.0 at first , decreased 10 % -60 % after 1 h of PDF , and then remained stable .
	manualset3
135529	2	406923	5	NULL	NULL	0	NULL	solutes 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sieving coefficients of different solutes ranged from 0.1 to 1.0 at first , decreased 10 % -60 % after 1 h of PDF , and then remained stable .
	manualset3
135530	3	406923	5	NULL	NULL	0	NULL	 0.1 to 1.0 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sieving coefficients of different solutes ranged from 0.1 to 1.0 at first , decreased 10 % -60 % after 1 h of PDF , and then remained stable .
	manualset3
135531	4	406923	5	NULL	NULL	0	NULL	10 % -60 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sieving coefficients of different solutes ranged from 0.1 to 1.0 at first , decreased 10 % -60 % after 1 h of PDF , and then remained stable .
	manualset3
135532	5	406923	5	NULL	NULL	0	NULL	1 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Sieving coefficients of different solutes ranged from 0.1 to 1.0 at first , decreased 10 % -60 % after 1 h of PDF , and then remained stable .
	manualset3
135533	6	406923	5	NULL	NULL	0	NULL	PDF 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sieving coefficients of different solutes ranged from 0.1 to 1.0 at first , decreased 10 % -60 % after 1 h of PDF , and then remained stable .
	manualset3
135534	1	406924	5	NULL	NULL	0	NULL	Sigma-hole bonding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sigma-hole bonding has been observed , experimentally and computationally , for many covalently-bonded atoms of Groups V-VII .
	manualset3
135535	2	406924	5	NULL	NULL	0	NULL	covalently-bonded atoms 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Sigma-hole bonding has been observed , experimentally and computationally , for many covalently-bonded atoms of Groups V-VII .
	manualset3
135536	3	406924	5	NULL	NULL	0	NULL	Groups V-VII	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Sigma-hole bonding has been observed , experimentally and computationally , for many covalently-bonded atoms of Groups V-VII .
	manualset3
135537	1	406925	5	NULL	NULL	0	NULL	Signal intensities 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Signal intensities clearly dependent on orientation were observed in the cortical and deep white matter of the brain and in the white matter of the spinal cord .
	manualset3
135538	2	406925	5	NULL	NULL	0	NULL	orientation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Signal intensities clearly dependent on orientation were observed in the cortical and deep white matter of the brain and in the white matter of the spinal cord .
	manualset3
135539	3	406925	5	NULL	NULL	0	NULL	cortical and deep white matter	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Signal intensities clearly dependent on orientation were observed in the cortical and deep white matter of the brain and in the white matter of the spinal cord .
	manualset3
135540	4	406925	5	NULL	NULL	0	NULL	brain 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Signal intensities clearly dependent on orientation were observed in the cortical and deep white matter of the brain and in the white matter of the spinal cord .
	manualset3
135541	5	406925	5	NULL	NULL	0	NULL	white matter 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Signal intensities clearly dependent on orientation were observed in the cortical and deep white matter of the brain and in the white matter of the spinal cord .
	manualset3
135542	6	406925	5	NULL	NULL	0	NULL	spinal cord	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Signal intensities clearly dependent on orientation were observed in the cortical and deep white matter of the brain and in the white matter of the spinal cord .
	manualset3
135543	1	406926	5	NULL	NULL	0	NULL	Signalling mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Signalling mechanisms involving cAMP have a well-documented role in the coordination of multicellular development and differentiation leading to spore formation in the social amoeba , Dictyostelium discoideum .
	manualset3
135544	2	406926	5	NULL	NULL	0	NULL	 cAMP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Signalling mechanisms involving cAMP have a well-documented role in the coordination of multicellular development and differentiation leading to spore formation in the social amoeba , Dictyostelium discoideum .
	manualset3
135545	3	406926	5	NULL	NULL	0	NULL	well-documented role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Signalling mechanisms involving cAMP have a well-documented role in the coordination of multicellular development and differentiation leading to spore formation in the social amoeba , Dictyostelium discoideum .
	manualset3
135546	4	406926	5	NULL	NULL	0	NULL	coordination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Signalling mechanisms involving cAMP have a well-documented role in the coordination of multicellular development and differentiation leading to spore formation in the social amoeba , Dictyostelium discoideum .
	manualset3
135547	5	406926	5	NULL	NULL	0	NULL	multicellular development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Signalling mechanisms involving cAMP have a well-documented role in the coordination of multicellular development and differentiation leading to spore formation in the social amoeba , Dictyostelium discoideum .
	manualset3
135548	6	406926	5	NULL	NULL	0	NULL	differentiation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Signalling mechanisms involving cAMP have a well-documented role in the coordination of multicellular development and differentiation leading to spore formation in the social amoeba , Dictyostelium discoideum .
	manualset3
135549	7	406926	5	NULL	NULL	0	NULL	spore formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Signalling mechanisms involving cAMP have a well-documented role in the coordination of multicellular development and differentiation leading to spore formation in the social amoeba , Dictyostelium discoideum .
	manualset3
135550	8	406926	5	NULL	NULL	0	NULL	social amoeba , Dictyostelium discoideum 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Signalling mechanisms involving cAMP have a well-documented role in the coordination of multicellular development and differentiation leading to spore formation in the social amoeba , Dictyostelium discoideum .
	manualset3
135551	1	406927	5	NULL	NULL	0	NULL	Signals 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Signals generated by hR could be identified using four criteria : wavelength dependence , Cl - dependence , shunting by valinomycin and K + , and the absence of these signals in hR-deficient mutants .
	manualset3
135552	2	406927	5	NULL	NULL	0	NULL	hR 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Signals generated by hR could be identified using four criteria : wavelength dependence , Cl - dependence , shunting by valinomycin and K + , and the absence of these signals in hR-deficient mutants .
	manualset3
135553	3	406927	5	NULL	NULL	0	NULL	four 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Signals generated by hR could be identified using four criteria : wavelength dependence , Cl - dependence , shunting by valinomycin and K + , and the absence of these signals in hR-deficient mutants .
	manualset3
135554	4	406927	5	NULL	NULL	NULL	NULL	criteria 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Signals generated by hR could be identified using four criteria : wavelength dependence , Cl - dependence , shunting by valinomycin and K + , and the absence of these signals in hR-deficient mutants .
	manualset3
135555	5	406927	5	NULL	NULL	0	NULL	wavelength dependence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Signals generated by hR could be identified using four criteria : wavelength dependence , Cl - dependence , shunting by valinomycin and K + , and the absence of these signals in hR-deficient mutants .
	manualset3
135556	6	406927	5	NULL	NULL	0	NULL	Cl - dependence 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Signals generated by hR could be identified using four criteria : wavelength dependence , Cl - dependence , shunting by valinomycin and K + , and the absence of these signals in hR-deficient mutants .
	manualset3
135557	7	406927	5	NULL	NULL	0	NULL	valinomycin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Signals generated by hR could be identified using four criteria : wavelength dependence , Cl - dependence , shunting by valinomycin and K + , and the absence of these signals in hR-deficient mutants .
	manualset3
135558	8	406927	5	NULL	NULL	0	NULL	K + 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Signals generated by hR could be identified using four criteria : wavelength dependence , Cl - dependence , shunting by valinomycin and K + , and the absence of these signals in hR-deficient mutants .
	manualset3
135559	9	406927	5	NULL	NULL	0	NULL	absence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Signals generated by hR could be identified using four criteria : wavelength dependence , Cl - dependence , shunting by valinomycin and K + , and the absence of these signals in hR-deficient mutants .
	manualset3
135560	10	406927	5	NULL	NULL	0	NULL	signals 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Signals generated by hR could be identified using four criteria : wavelength dependence , Cl - dependence , shunting by valinomycin and K + , and the absence of these signals in hR-deficient mutants .
	manualset3
135561	11	406927	5	NULL	NULL	0	NULL	hR-deficient mutants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Signals generated by hR could be identified using four criteria : wavelength dependence , Cl - dependence , shunting by valinomycin and K + , and the absence of these signals in hR-deficient mutants .
	manualset3
135562	1	406928	5	NULL	NULL	0	NULL	Significance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Significance of bronchologic examination in the prevention of chronic bronchial lesions ) .
	manualset3
135563	2	406928	5	NULL	NULL	0	NULL	bronchologic examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Significance of bronchologic examination in the prevention of chronic bronchial lesions ) .
	manualset3
135564	3	406928	5	NULL	NULL	0	NULL	prevention 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Significance of bronchologic examination in the prevention of chronic bronchial lesions ) .
	manualset3
135565	4	406928	5	NULL	NULL	0	NULL	chronic bronchial lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Significance of bronchologic examination in the prevention of chronic bronchial lesions ) .
	manualset3
135566	1	406929	5	NULL	NULL	0	NULL	novel candidate	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel candidate cis-regulatory motif pair in the promoters of germline and oogenesis genes in C. elegans .
	manualset3
135567	2	406929	5	NULL	NULL	0	NULL	cis-regulatory motif pair	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel candidate cis-regulatory motif pair in the promoters of germline and oogenesis genes in C. elegans .
	manualset3
135568	3	406929	5	NULL	NULL	0	NULL	promoters 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel candidate cis-regulatory motif pair in the promoters of germline and oogenesis genes in C. elegans .
	manualset3
135569	4	406929	5	NULL	NULL	0	NULL	germline genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel candidate cis-regulatory motif pair in the promoters of germline and oogenesis genes in C. elegans .
	manualset3
135570	5	406929	5	NULL	NULL	0	NULL	oogenesis genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel candidate cis-regulatory motif pair in the promoters of germline and oogenesis genes in C. elegans .
	manualset3
135571	6	406929	5	NULL	NULL	0	NULL	C. elegans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel candidate cis-regulatory motif pair in the promoters of germline and oogenesis genes in C. elegans .
	manualset3
135572	1	406930	5	NULL	NULL	0	NULL	Significance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Significance of ionic fluxes and changes in membrane potential for stimulus-secretion coupling in pancreatic B-cells .
	manualset3
135573	2	406930	5	NULL	NULL	0	NULL	ionic fluxes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Significance of ionic fluxes and changes in membrane potential for stimulus-secretion coupling in pancreatic B-cells .
	manualset3
135574	3	406930	5	NULL	NULL	0	NULL	changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Significance of ionic fluxes and changes in membrane potential for stimulus-secretion coupling in pancreatic B-cells .
	manualset3
135575	4	406930	5	NULL	NULL	0	NULL	membrane potential	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Significance of ionic fluxes and changes in membrane potential for stimulus-secretion coupling in pancreatic B-cells .
	manualset3
135576	5	406930	5	NULL	NULL	0	NULL	stimulus-secretion coupling 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Significance of ionic fluxes and changes in membrane potential for stimulus-secretion coupling in pancreatic B-cells .
	manualset3
135577	6	406930	5	NULL	NULL	0	NULL	pancreatic B-cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Significance of ionic fluxes and changes in membrane potential for stimulus-secretion coupling in pancreatic B-cells .
	manualset3
135721	1	406931	5	NULL	NULL	0	NULL	 Target x Condition interactions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant Target x Condition interactions were obtained on measures of perceived age , competence , and memory ability .
	manualset3
135722	2	406931	5	NULL	NULL	0	NULL	measures 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant Target x Condition interactions were obtained on measures of perceived age , competence , and memory ability .
	manualset3
135723	3	406931	5	NULL	NULL	0	NULL	perceived age	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant Target x Condition interactions were obtained on measures of perceived age , competence , and memory ability .
	manualset3
135724	4	406931	5	NULL	NULL	0	NULL	competence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant Target x Condition interactions were obtained on measures of perceived age , competence , and memory ability .
	manualset3
135725	5	406931	5	NULL	NULL	0	NULL	memory ability	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant Target x Condition interactions were obtained on measures of perceived age , competence , and memory ability .
	manualset3
135726	1	406932	5	NULL	NULL	0	NULL	amounts 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant amounts of sIL-5R alpha were detected in sera and ascitic fluids of mice bearing tumors ( BCL1 and MOPC104E ) that responded to IL-5 for DNA synthesis , but not in sera of normal mice .
	manualset3
135727	2	406932	5	NULL	NULL	0	NULL	sIL-5R alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant amounts of sIL-5R alpha were detected in sera and ascitic fluids of mice bearing tumors ( BCL1 and MOPC104E ) that responded to IL-5 for DNA synthesis , but not in sera of normal mice .
	manualset3
135728	3	406932	5	NULL	NULL	0	NULL	sera 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant amounts of sIL-5R alpha were detected in sera and ascitic fluids of mice bearing tumors ( BCL1 and MOPC104E ) that responded to IL-5 for DNA synthesis , but not in sera of normal mice .
	manualset3
135729	4	406932	5	NULL	NULL	0	NULL	ascitic fluids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant amounts of sIL-5R alpha were detected in sera and ascitic fluids of mice bearing tumors ( BCL1 and MOPC104E ) that responded to IL-5 for DNA synthesis , but not in sera of normal mice .
	manualset3
135730	5	406932	5	NULL	NULL	0	NULL	mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant amounts of sIL-5R alpha were detected in sera and ascitic fluids of mice bearing tumors ( BCL1 and MOPC104E ) that responded to IL-5 for DNA synthesis , but not in sera of normal mice .
	manualset3
135731	6	406932	5	NULL	NULL	0	NULL	tumors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant amounts of sIL-5R alpha were detected in sera and ascitic fluids of mice bearing tumors ( BCL1 and MOPC104E ) that responded to IL-5 for DNA synthesis , but not in sera of normal mice .
	manualset3
135732	7	406932	5	NULL	NULL	0	NULL	BCL1 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant amounts of sIL-5R alpha were detected in sera and ascitic fluids of mice bearing tumors ( BCL1 and MOPC104E ) that responded to IL-5 for DNA synthesis , but not in sera of normal mice .
	manualset3
135733	8	406932	5	NULL	NULL	0	NULL	MOPC104E 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant amounts of sIL-5R alpha were detected in sera and ascitic fluids of mice bearing tumors ( BCL1 and MOPC104E ) that responded to IL-5 for DNA synthesis , but not in sera of normal mice .
	manualset3
135734	9	406932	5	NULL	NULL	0	NULL	IL-5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant amounts of sIL-5R alpha were detected in sera and ascitic fluids of mice bearing tumors ( BCL1 and MOPC104E ) that responded to IL-5 for DNA synthesis , but not in sera of normal mice .
	manualset3
135735	10	406932	5	NULL	NULL	0	NULL	DNA synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant amounts of sIL-5R alpha were detected in sera and ascitic fluids of mice bearing tumors ( BCL1 and MOPC104E ) that responded to IL-5 for DNA synthesis , but not in sera of normal mice .
	manualset3
135736	11	406932	5	NULL	NULL	0	NULL	sera 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant amounts of sIL-5R alpha were detected in sera and ascitic fluids of mice bearing tumors ( BCL1 and MOPC104E ) that responded to IL-5 for DNA synthesis , but not in sera of normal mice .
	manualset3
135737	12	406932	5	NULL	NULL	0	NULL	normal mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant amounts of sIL-5R alpha were detected in sera and ascitic fluids of mice bearing tumors ( BCL1 and MOPC104E ) that responded to IL-5 for DNA synthesis , but not in sera of normal mice .
	manualset3
135738	1	406933	5	NULL	NULL	0	NULL	complications 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant complications occurred in 74 procedures ( 0.81 % ) , with 32 ( 1.24 % ) complications with MC and 42 ( 0.64 % ) with VCD ( p = 0.004 ) .
	manualset3
135739	2	406933	5	NULL	NULL	0	NULL	74 procedures ( 0.81 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant complications occurred in 74 procedures ( 0.81 % ) , with 32 ( 1.24 % ) complications with MC and 42 ( 0.64 % ) with VCD ( p = 0.004 ) .
	manualset3
135740	3	406933	5	NULL	NULL	0	NULL	32 ( 1.24 % ) complications 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant complications occurred in 74 procedures ( 0.81 % ) , with 32 ( 1.24 % ) complications with MC and 42 ( 0.64 % ) with VCD ( p = 0.004 ) .
	manualset3
135741	4	406933	5	NULL	NULL	0	NULL	MC 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant complications occurred in 74 procedures ( 0.81 % ) , with 32 ( 1.24 % ) complications with MC and 42 ( 0.64 % ) with VCD ( p = 0.004 ) .
	manualset3
135742	5	406933	5	NULL	NULL	0	NULL	42 ( 0.64 % ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant complications occurred in 74 procedures ( 0.81 % ) , with 32 ( 1.24 % ) complications with MC and 42 ( 0.64 % ) with VCD ( p = 0.004 ) .
	manualset3
135743	6	406933	5	NULL	NULL	0	NULL	VCD 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant complications occurred in 74 procedures ( 0.81 % ) , with 32 ( 1.24 % ) complications with MC and 42 ( 0.64 % ) with VCD ( p = 0.004 ) .
	manualset3
135744	7	406933	5	NULL	NULL	0	NULL	 p = 0.004 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant complications occurred in 74 procedures ( 0.81 % ) , with 32 ( 1.24 % ) complications with MC and 42 ( 0.64 % ) with VCD ( p = 0.004 ) .
	manualset3
135745	1	406934	5	NULL	NULL	0	NULL	decrease 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant decrease in angiopoietin-1 and angiopoietin-2 after radical prostatectomy in prostate cancer patients .
	manualset3
135746	2	406934	5	NULL	NULL	0	NULL	angiopoietin-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant decrease in angiopoietin-1 and angiopoietin-2 after radical prostatectomy in prostate cancer patients .
	manualset3
135747	3	406934	5	NULL	NULL	0	NULL	angiopoietin-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant decrease in angiopoietin-1 and angiopoietin-2 after radical prostatectomy in prostate cancer patients .
	manualset3
135748	4	406934	5	NULL	NULL	0	NULL	radical prostatectomy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant decrease in angiopoietin-1 and angiopoietin-2 after radical prostatectomy in prostate cancer patients .
	manualset3
135749	5	406934	5	NULL	NULL	0	NULL	prostate cancer patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant decrease in angiopoietin-1 and angiopoietin-2 after radical prostatectomy in prostate cancer patients .
	manualset3
135750	1	406935	5	NULL	NULL	0	NULL	Significant differences 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant differences in pre - and post-module scores suggest that the course had significant impact on attitudes toward early diagnosis , treatment aggressiveness , and acceptance of death .
	manualset3
135751	2	406935	5	NULL	NULL	0	NULL	pre -module scores 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant differences in pre - and post-module scores suggest that the course had significant impact on attitudes toward early diagnosis , treatment aggressiveness , and acceptance of death .
	manualset3
135752	3	406935	5	NULL	NULL	0	NULL	post-module scores 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant differences in pre - and post-module scores suggest that the course had significant impact on attitudes toward early diagnosis , treatment aggressiveness , and acceptance of death .
	manualset3
135753	4	406935	5	NULL	NULL	0	NULL	course 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant differences in pre - and post-module scores suggest that the course had significant impact on attitudes toward early diagnosis , treatment aggressiveness , and acceptance of death .
	manualset3
135754	5	406935	5	NULL	NULL	0	NULL	significant impact 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant differences in pre - and post-module scores suggest that the course had significant impact on attitudes toward early diagnosis , treatment aggressiveness , and acceptance of death .
	manualset3
135755	6	406935	5	NULL	NULL	0	NULL	attitudes 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant differences in pre - and post-module scores suggest that the course had significant impact on attitudes toward early diagnosis , treatment aggressiveness , and acceptance of death .
	manualset3
135756	7	406935	5	NULL	NULL	0	NULL	early diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant differences in pre - and post-module scores suggest that the course had significant impact on attitudes toward early diagnosis , treatment aggressiveness , and acceptance of death .
	manualset3
135757	8	406935	5	NULL	NULL	0	NULL	treatment aggressiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant differences in pre - and post-module scores suggest that the course had significant impact on attitudes toward early diagnosis , treatment aggressiveness , and acceptance of death .
	manualset3
135758	9	406935	5	NULL	NULL	0	NULL	acceptance 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant differences in pre - and post-module scores suggest that the course had significant impact on attitudes toward early diagnosis , treatment aggressiveness , and acceptance of death .
	manualset3
135759	10	406935	5	NULL	NULL	0	NULL	death 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant differences in pre - and post-module scores suggest that the course had significant impact on attitudes toward early diagnosis , treatment aggressiveness , and acceptance of death .
	manualset3
135760	1	406936	5	NULL	NULL	0	NULL	down-regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant down-regulation of alpha-albumin in human hepatoma and its implication .
	manualset3
135761	2	406936	5	NULL	NULL	0	NULL	alpha-albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant down-regulation of alpha-albumin in human hepatoma and its implication .
	manualset3
135762	3	406936	5	NULL	NULL	0	NULL	human hepatoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant down-regulation of alpha-albumin in human hepatoma and its implication .
	manualset3
135763	4	406936	5	NULL	NULL	0	NULL	implication 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant down-regulation of alpha-albumin in human hepatoma and its implication .
	manualset3
135764	1	406937	5	NULL	NULL	0	NULL	novel class of acetylferrocene-derived Schiff-bases	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel class of acetylferrocene-derived Schiff-bases such as 2-pyrazinoyl-1 - ( 2-ferroceneylmethylene ) - hydrazide ( HL ( 1 ) ) and 2-nicotinoyl-1 - ( 2-ferrocenylmethylene ) hydrazide ( HL ( 2 ) ) have been synthesized and characterized by their IR , ( 1 ) H NMR , ( 13 ) C NMR and microanalytical date .
	manualset3
135765	2	406937	5	NULL	NULL	0	NULL	2-pyrazinoyl-1 - ( 2-ferroceneylmethylene ) - hydrazide ( HL ( 1 ) )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel class of acetylferrocene-derived Schiff-bases such as 2-pyrazinoyl-1 - ( 2-ferroceneylmethylene ) - hydrazide ( HL ( 1 ) ) and 2-nicotinoyl-1 - ( 2-ferrocenylmethylene ) hydrazide ( HL ( 2 ) ) have been synthesized and characterized by their IR , ( 1 ) H NMR , ( 13 ) C NMR and microanalytical date .
	manualset3
135766	3	406937	5	NULL	NULL	0	NULL	 2-nicotinoyl-1 - ( 2-ferrocenylmethylene ) hydrazide ( HL ( 2 ) )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel class of acetylferrocene-derived Schiff-bases such as 2-pyrazinoyl-1 - ( 2-ferroceneylmethylene ) - hydrazide ( HL ( 1 ) ) and 2-nicotinoyl-1 - ( 2-ferrocenylmethylene ) hydrazide ( HL ( 2 ) ) have been synthesized and characterized by their IR , ( 1 ) H NMR , ( 13 ) C NMR and microanalytical date .
	manualset3
135767	4	406937	5	NULL	NULL	0	NULL	IR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel class of acetylferrocene-derived Schiff-bases such as 2-pyrazinoyl-1 - ( 2-ferroceneylmethylene ) - hydrazide ( HL ( 1 ) ) and 2-nicotinoyl-1 - ( 2-ferrocenylmethylene ) hydrazide ( HL ( 2 ) ) have been synthesized and characterized by their IR , ( 1 ) H NMR , ( 13 ) C NMR and microanalytical date .
	manualset3
135768	5	406937	5	NULL	NULL	0	NULL	H NMR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel class of acetylferrocene-derived Schiff-bases such as 2-pyrazinoyl-1 - ( 2-ferroceneylmethylene ) - hydrazide ( HL ( 1 ) ) and 2-nicotinoyl-1 - ( 2-ferrocenylmethylene ) hydrazide ( HL ( 2 ) ) have been synthesized and characterized by their IR , ( 1 ) H NMR , ( 13 ) C NMR and microanalytical date .
	manualset3
135769	6	406937	5	NULL	NULL	0	NULL	C NMR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel class of acetylferrocene-derived Schiff-bases such as 2-pyrazinoyl-1 - ( 2-ferroceneylmethylene ) - hydrazide ( HL ( 1 ) ) and 2-nicotinoyl-1 - ( 2-ferrocenylmethylene ) hydrazide ( HL ( 2 ) ) have been synthesized and characterized by their IR , ( 1 ) H NMR , ( 13 ) C NMR and microanalytical date .
	manualset3
135770	7	406937	5	NULL	NULL	0	NULL	microanalytical date	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel class of acetylferrocene-derived Schiff-bases such as 2-pyrazinoyl-1 - ( 2-ferroceneylmethylene ) - hydrazide ( HL ( 1 ) ) and 2-nicotinoyl-1 - ( 2-ferrocenylmethylene ) hydrazide ( HL ( 2 ) ) have been synthesized and characterized by their IR , ( 1 ) H NMR , ( 13 ) C NMR and microanalytical date .
	manualset3
135771	1	406938	5	NULL	NULL	0	NULL	improvement 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant improvement in both subjective and objective voice measures was achieved after surgical removal of the lingual thyroid gland , which allowed for maintenance of a consistent euthyroid state .
	manualset3
135772	2	406938	5	NULL	NULL	0	NULL	subjective voice measures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant improvement in both subjective and objective voice measures was achieved after surgical removal of the lingual thyroid gland , which allowed for maintenance of a consistent euthyroid state .
	manualset3
135773	3	406938	5	NULL	NULL	0	NULL	objective voice measures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant improvement in both subjective and objective voice measures was achieved after surgical removal of the lingual thyroid gland , which allowed for maintenance of a consistent euthyroid state .
	manualset3
135774	4	406938	5	NULL	NULL	0	NULL	surgical removal 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant improvement in both subjective and objective voice measures was achieved after surgical removal of the lingual thyroid gland , which allowed for maintenance of a consistent euthyroid state .
	manualset3
135775	5	406938	5	NULL	NULL	0	NULL	lingual thyroid gland	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant improvement in both subjective and objective voice measures was achieved after surgical removal of the lingual thyroid gland , which allowed for maintenance of a consistent euthyroid state .
	manualset3
135776	6	406938	5	NULL	NULL	0	NULL	maintenance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant improvement in both subjective and objective voice measures was achieved after surgical removal of the lingual thyroid gland , which allowed for maintenance of a consistent euthyroid state .
	manualset3
135777	7	406938	5	NULL	NULL	0	NULL	consistent euthyroid state	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant improvement in both subjective and objective voice measures was achieved after surgical removal of the lingual thyroid gland , which allowed for maintenance of a consistent euthyroid state .
	manualset3
135778	1	406939	5	NULL	NULL	0	NULL	improvements 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant improvements in subject-assessed nasal congestion scores ( P & lt ; 0.01 ) and rhinomanometry ( P = 0.036 ) were noted with L/M as compared with placebo .
	manualset3
135779	2	406939	5	NULL	NULL	0	NULL	subject-assessed nasal congestion scores	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant improvements in subject-assessed nasal congestion scores ( P & lt ; 0.01 ) and rhinomanometry ( P = 0.036 ) were noted with L/M as compared with placebo .
	manualset3
135780	3	406939	5	NULL	NULL	0	NULL	p & lt ; 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant improvements in subject-assessed nasal congestion scores ( P & lt ; 0.01 ) and rhinomanometry ( P = 0.036 ) were noted with L/M as compared with placebo .
	manualset3
135781	4	406939	5	NULL	NULL	0	NULL	rhinomanometry 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant improvements in subject-assessed nasal congestion scores ( P & lt ; 0.01 ) and rhinomanometry ( P = 0.036 ) were noted with L/M as compared with placebo .
	manualset3
135782	5	406939	5	NULL	NULL	0	NULL	P = 0.036	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant improvements in subject-assessed nasal congestion scores ( P & lt ; 0.01 ) and rhinomanometry ( P = 0.036 ) were noted with L/M as compared with placebo .
	manualset3
135783	6	406939	5	NULL	NULL	0	NULL	L/M 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant improvements in subject-assessed nasal congestion scores ( P & lt ; 0.01 ) and rhinomanometry ( P = 0.036 ) were noted with L/M as compared with placebo .
	manualset3
135784	7	406939	5	NULL	NULL	0	NULL	placebo 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant improvements in subject-assessed nasal congestion scores ( P & lt ; 0.01 ) and rhinomanometry ( P = 0.036 ) were noted with L/M as compared with placebo .
	manualset3
135785	1	406940	5	NULL	NULL	0	NULL	levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant levels of Fc epsilon RIIb expression were obtained after 12 h of incubation with IL-4 and maximal expression was observed between 24 to 48 h after which the expression declined .
	manualset3
135786	2	406940	5	NULL	NULL	0	NULL	Fc epsilon RIIb expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant levels of Fc epsilon RIIb expression were obtained after 12 h of incubation with IL-4 and maximal expression was observed between 24 to 48 h after which the expression declined .
	manualset3
135787	3	406940	5	NULL	NULL	0	NULL	12 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant levels of Fc epsilon RIIb expression were obtained after 12 h of incubation with IL-4 and maximal expression was observed between 24 to 48 h after which the expression declined .
	manualset3
135788	4	406940	5	NULL	NULL	0	NULL	incubation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant levels of Fc epsilon RIIb expression were obtained after 12 h of incubation with IL-4 and maximal expression was observed between 24 to 48 h after which the expression declined .
	manualset3
135789	5	406940	5	NULL	NULL	0	NULL	IL-4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant levels of Fc epsilon RIIb expression were obtained after 12 h of incubation with IL-4 and maximal expression was observed between 24 to 48 h after which the expression declined .
	manualset3
135790	6	406940	5	NULL	NULL	0	NULL	maximal expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant levels of Fc epsilon RIIb expression were obtained after 12 h of incubation with IL-4 and maximal expression was observed between 24 to 48 h after which the expression declined .
	manualset3
135791	7	406940	5	NULL	NULL	0	NULL	24 to 48 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant levels of Fc epsilon RIIb expression were obtained after 12 h of incubation with IL-4 and maximal expression was observed between 24 to 48 h after which the expression declined .
	manualset3
135792	8	406940	5	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant levels of Fc epsilon RIIb expression were obtained after 12 h of incubation with IL-4 and maximal expression was observed between 24 to 48 h after which the expression declined .
	manualset3
135793	1	406941	5	NULL	NULL	0	NULL	positive correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant positive correlation was found between both ( ONc ) latency and ONc-L1 interpeak latency and body height ( H ) .
	manualset3
135794	2	406941	5	NULL	NULL	0	NULL	 ( ONc ) latency	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant positive correlation was found between both ( ONc ) latency and ONc-L1 interpeak latency and body height ( H ) .
	manualset3
135795	3	406941	5	NULL	NULL	0	NULL	ONc-L1 interpeak latency	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant positive correlation was found between both ( ONc ) latency and ONc-L1 interpeak latency and body height ( H ) .
	manualset3
135796	4	406941	5	NULL	NULL	0	NULL	body height ( H )	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant positive correlation was found between both ( ONc ) latency and ONc-L1 interpeak latency and body height ( H ) .
	manualset3
135797	1	406942	5	NULL	NULL	0	NULL	prognostic factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant prognostic factors in Stage II were the value of hemoglobin ( p = 0.0115 ) and age ( p = 0.0431 ) by logrank test .
	manualset3
135798	2	406942	5	NULL	NULL	0	NULL	Stage II 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant prognostic factors in Stage II were the value of hemoglobin ( p = 0.0115 ) and age ( p = 0.0431 ) by logrank test .
	manualset3
135799	3	406942	5	NULL	NULL	0	NULL	value 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant prognostic factors in Stage II were the value of hemoglobin ( p = 0.0115 ) and age ( p = 0.0431 ) by logrank test .
	manualset3
135800	4	406942	5	NULL	NULL	0	NULL	hemoglobin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant prognostic factors in Stage II were the value of hemoglobin ( p = 0.0115 ) and age ( p = 0.0431 ) by logrank test .
	manualset3
135801	5	406942	5	NULL	NULL	0	NULL	p = 0.0115	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant prognostic factors in Stage II were the value of hemoglobin ( p = 0.0115 ) and age ( p = 0.0431 ) by logrank test .
	manualset3
135802	6	406942	5	NULL	NULL	0	NULL	age 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant prognostic factors in Stage II were the value of hemoglobin ( p = 0.0115 ) and age ( p = 0.0431 ) by logrank test .
	manualset3
135803	7	406942	5	NULL	NULL	0	NULL	p = 0.0431	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant prognostic factors in Stage II were the value of hemoglobin ( p = 0.0115 ) and age ( p = 0.0431 ) by logrank test .
	manualset3
135804	8	406942	5	NULL	NULL	0	NULL	logrank test 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant prognostic factors in Stage II were the value of hemoglobin ( p = 0.0115 ) and age ( p = 0.0431 ) by logrank test .
	manualset3
135805	1	406943	5	NULL	NULL	0	NULL	reductions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant reductions in blood pressure were attained between baseline and the 3-month evaluation ( P & lt ; 0.001 ) and these changes remained at the 3-year follow-up in both systolic BP of -15.4 + / - 18.7 mm Hg and diastolic BP of -10.3 + / - 10.0 mm Hg .
	manualset3
135806	2	406943	5	NULL	NULL	0	NULL	blood pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant reductions in blood pressure were attained between baseline and the 3-month evaluation ( P & lt ; 0.001 ) and these changes remained at the 3-year follow-up in both systolic BP of -15.4 + / - 18.7 mm Hg and diastolic BP of -10.3 + / - 10.0 mm Hg .
	manualset3
135807	3	406943	5	NULL	NULL	0	NULL	baseline 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant reductions in blood pressure were attained between baseline and the 3-month evaluation ( P & lt ; 0.001 ) and these changes remained at the 3-year follow-up in both systolic BP of -15.4 + / - 18.7 mm Hg and diastolic BP of -10.3 + / - 10.0 mm Hg .
	manualset3
135808	4	406943	5	NULL	NULL	0	NULL	3-month evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant reductions in blood pressure were attained between baseline and the 3-month evaluation ( P & lt ; 0.001 ) and these changes remained at the 3-year follow-up in both systolic BP of -15.4 + / - 18.7 mm Hg and diastolic BP of -10.3 + / - 10.0 mm Hg .
	manualset3
135809	5	406943	5	NULL	NULL	0	NULL	 P & lt ; 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant reductions in blood pressure were attained between baseline and the 3-month evaluation ( P & lt ; 0.001 ) and these changes remained at the 3-year follow-up in both systolic BP of -15.4 + / - 18.7 mm Hg and diastolic BP of -10.3 + / - 10.0 mm Hg .
	manualset3
135810	6	406943	5	NULL	NULL	0	NULL	changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant reductions in blood pressure were attained between baseline and the 3-month evaluation ( P & lt ; 0.001 ) and these changes remained at the 3-year follow-up in both systolic BP of -15.4 + / - 18.7 mm Hg and diastolic BP of -10.3 + / - 10.0 mm Hg .
	manualset3
135811	7	406943	5	NULL	NULL	0	NULL	 3-year follow-up	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant reductions in blood pressure were attained between baseline and the 3-month evaluation ( P & lt ; 0.001 ) and these changes remained at the 3-year follow-up in both systolic BP of -15.4 + / - 18.7 mm Hg and diastolic BP of -10.3 + / - 10.0 mm Hg .
	manualset3
135812	8	406943	5	NULL	NULL	0	NULL	systolic BP	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant reductions in blood pressure were attained between baseline and the 3-month evaluation ( P & lt ; 0.001 ) and these changes remained at the 3-year follow-up in both systolic BP of -15.4 + / - 18.7 mm Hg and diastolic BP of -10.3 + / - 10.0 mm Hg .
	manualset3
135813	9	406943	5	NULL	NULL	0	NULL	-15.4 + / - 18.7 mm Hg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant reductions in blood pressure were attained between baseline and the 3-month evaluation ( P & lt ; 0.001 ) and these changes remained at the 3-year follow-up in both systolic BP of -15.4 + / - 18.7 mm Hg and diastolic BP of -10.3 + / - 10.0 mm Hg .
	manualset3
135814	10	406943	5	NULL	NULL	0	NULL	diastolic BP	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant reductions in blood pressure were attained between baseline and the 3-month evaluation ( P & lt ; 0.001 ) and these changes remained at the 3-year follow-up in both systolic BP of -15.4 + / - 18.7 mm Hg and diastolic BP of -10.3 + / - 10.0 mm Hg .
	manualset3
135910	11	406943	5	NULL	NULL	0	NULL	-10.3 + / - 10.0 mm Hg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant reductions in blood pressure were attained between baseline and the 3-month evaluation ( P & lt ; 0.001 ) and these changes remained at the 3-year follow-up in both systolic BP of -15.4 + / - 18.7 mm Hg and diastolic BP of -10.3 + / - 10.0 mm Hg .
	manualset3
135912	1	406944	5	NULL	NULL	0	NULL	reductions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant reductions in intersegmental joint forces and moments were observed in the operated hindlimb one month after surgery , although kinematic gait parameters were unaltered .
	manualset3
135913	2	406944	5	NULL	NULL	0	NULL	intersegmental joint forces 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant reductions in intersegmental joint forces and moments were observed in the operated hindlimb one month after surgery , although kinematic gait parameters were unaltered .
	manualset3
135914	3	406944	5	NULL	NULL	0	NULL	moments 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant reductions in intersegmental joint forces and moments were observed in the operated hindlimb one month after surgery , although kinematic gait parameters were unaltered .
	manualset3
135916	4	406944	5	NULL	NULL	0	NULL	operated hindlimb	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant reductions in intersegmental joint forces and moments were observed in the operated hindlimb one month after surgery , although kinematic gait parameters were unaltered .
	manualset3
135918	5	406944	5	NULL	NULL	0	NULL	one month 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant reductions in intersegmental joint forces and moments were observed in the operated hindlimb one month after surgery , although kinematic gait parameters were unaltered .
	manualset3
135921	6	406944	5	NULL	NULL	0	NULL	surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant reductions in intersegmental joint forces and moments were observed in the operated hindlimb one month after surgery , although kinematic gait parameters were unaltered .
	manualset3
135922	7	406944	5	NULL	NULL	0	NULL	kinematic gait parameters 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant reductions in intersegmental joint forces and moments were observed in the operated hindlimb one month after surgery , although kinematic gait parameters were unaltered .
	manualset3
135939	1	406945	5	NULL	NULL	0	NULL	self-selection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant self-selection was observed among outdoor workers , whereby people with fair or medium complexions and a tendency to sunburn were systematically underrepresented among those in long-term outdoor occupations although they accounted for more than 80 percent of the community study sample .
	manualset3
135940	2	406945	5	NULL	NULL	0	NULL	outdoor workers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant self-selection was observed among outdoor workers , whereby people with fair or medium complexions and a tendency to sunburn were systematically underrepresented among those in long-term outdoor occupations although they accounted for more than 80 percent of the community study sample .
	manualset3
135941	3	406945	5	NULL	NULL	0	NULL	people 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant self-selection was observed among outdoor workers , whereby people with fair or medium complexions and a tendency to sunburn were systematically underrepresented among those in long-term outdoor occupations although they accounted for more than 80 percent of the community study sample .
	manualset3
135942	4	406945	5	NULL	NULL	0	NULL	fair or medium complexions	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant self-selection was observed among outdoor workers , whereby people with fair or medium complexions and a tendency to sunburn were systematically underrepresented among those in long-term outdoor occupations although they accounted for more than 80 percent of the community study sample .
	manualset3
135943	5	406945	5	NULL	NULL	0	NULL	tendency 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant self-selection was observed among outdoor workers , whereby people with fair or medium complexions and a tendency to sunburn were systematically underrepresented among those in long-term outdoor occupations although they accounted for more than 80 percent of the community study sample .
	manualset3
135944	6	406945	5	NULL	NULL	0	NULL	sunburn 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant self-selection was observed among outdoor workers , whereby people with fair or medium complexions and a tendency to sunburn were systematically underrepresented among those in long-term outdoor occupations although they accounted for more than 80 percent of the community study sample .
	manualset3
135945	7	406945	5	NULL	NULL	0	NULL	 long-term outdoor occupations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant self-selection was observed among outdoor workers , whereby people with fair or medium complexions and a tendency to sunburn were systematically underrepresented among those in long-term outdoor occupations although they accounted for more than 80 percent of the community study sample .
	manualset3
135946	8	406945	5	NULL	NULL	0	NULL	80 percent 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant self-selection was observed among outdoor workers , whereby people with fair or medium complexions and a tendency to sunburn were systematically underrepresented among those in long-term outdoor occupations although they accounted for more than 80 percent of the community study sample .
	manualset3
135947	9	406945	5	NULL	NULL	0	NULL	community study sample	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant self-selection was observed among outdoor workers , whereby people with fair or medium complexions and a tendency to sunburn were systematically underrepresented among those in long-term outdoor occupations although they accounted for more than 80 percent of the community study sample .
	manualset3
135948	1	406946	5	NULL	NULL	0	NULL	novel endo-type beta-agarase gene , agaA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel endo-type beta-agarase gene , agaA , was cloned from a newly isolated marine bacterium , Agarivorans sp .
	manualset3
135949	2	406946	5	NULL	NULL	0	NULL	marine bacterium , Agarivorans sp	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel endo-type beta-agarase gene , agaA , was cloned from a newly isolated marine bacterium , Agarivorans sp .
	manualset3
135950	1	406947	5	NULL	NULL	0	NULL	sex x trait anger interactions 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant sex x trait anger interactions were obtained for systolic blood pressure , diastolic blood pressure , and mean arterial pressure in which trait anger was negatively related to blood pressure decline for men but not for women .
	manualset3
135951	2	406947	5	NULL	NULL	0	NULL	systolic blood pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant sex x trait anger interactions were obtained for systolic blood pressure , diastolic blood pressure , and mean arterial pressure in which trait anger was negatively related to blood pressure decline for men but not for women .
	manualset3
135952	3	406947	5	NULL	NULL	0	NULL	diastolic blood pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant sex x trait anger interactions were obtained for systolic blood pressure , diastolic blood pressure , and mean arterial pressure in which trait anger was negatively related to blood pressure decline for men but not for women .
	manualset3
135953	4	406947	5	NULL	NULL	0	NULL	mean arterial pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant sex x trait anger interactions were obtained for systolic blood pressure , diastolic blood pressure , and mean arterial pressure in which trait anger was negatively related to blood pressure decline for men but not for women .
	manualset3
135954	5	406947	5	NULL	NULL	0	NULL	trait anger	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant sex x trait anger interactions were obtained for systolic blood pressure , diastolic blood pressure , and mean arterial pressure in which trait anger was negatively related to blood pressure decline for men but not for women .
	manualset3
135955	6	406947	5	NULL	NULL	0	NULL	blood pressure decline	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant sex x trait anger interactions were obtained for systolic blood pressure , diastolic blood pressure , and mean arterial pressure in which trait anger was negatively related to blood pressure decline for men but not for women .
	manualset3
135956	7	406947	5	NULL	NULL	0	NULL	men 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant sex x trait anger interactions were obtained for systolic blood pressure , diastolic blood pressure , and mean arterial pressure in which trait anger was negatively related to blood pressure decline for men but not for women .
	manualset3
135957	8	406947	5	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant sex x trait anger interactions were obtained for systolic blood pressure , diastolic blood pressure , and mean arterial pressure in which trait anger was negatively related to blood pressure decline for men but not for women .
	manualset3
135958	1	406948	5	NULL	NULL	0	NULL	therapeutic effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant therapeutic effects of these vectors do not only rely on tumor targeting but also on efficient release of viral progeny from host cells .
	manualset3
135959	2	406948	5	NULL	NULL	0	NULL	vectors 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant therapeutic effects of these vectors do not only rely on tumor targeting but also on efficient release of viral progeny from host cells .
	manualset3
135960	3	406948	5	NULL	NULL	0	NULL	tumor targeting	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant therapeutic effects of these vectors do not only rely on tumor targeting but also on efficient release of viral progeny from host cells .
	manualset3
135961	4	406948	5	NULL	NULL	0	NULL	viral progeny	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant therapeutic effects of these vectors do not only rely on tumor targeting but also on efficient release of viral progeny from host cells .
	manualset3
135962	5	406948	5	NULL	NULL	0	NULL	host cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant therapeutic effects of these vectors do not only rely on tumor targeting but also on efficient release of viral progeny from host cells .
	manualset3
138427	6	406948	5	NULL	NULL	0	NULL	release 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant therapeutic effects of these vectors do not only rely on tumor targeting but also on efficient release of viral progeny from host cells .
	manualset3
135963	1	406949	5	NULL	NULL	0	NULL	 P & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Significantly ( P & lt ; 0.05 ) lower values of TBARS , peroxide values , and hexanal contents were obtained for GK treated samples compared with cooked pork without antioxidant during refrigerated storage .
	manualset3
135964	2	406949	5	NULL	NULL	0	NULL	lower values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significantly ( P & lt ; 0.05 ) lower values of TBARS , peroxide values , and hexanal contents were obtained for GK treated samples compared with cooked pork without antioxidant during refrigerated storage .
	manualset3
135965	3	406949	5	NULL	NULL	0	NULL	TBARS 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significantly ( P & lt ; 0.05 ) lower values of TBARS , peroxide values , and hexanal contents were obtained for GK treated samples compared with cooked pork without antioxidant during refrigerated storage .
	manualset3
135966	4	406949	5	NULL	NULL	0	NULL	peroxide values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significantly ( P & lt ; 0.05 ) lower values of TBARS , peroxide values , and hexanal contents were obtained for GK treated samples compared with cooked pork without antioxidant during refrigerated storage .
	manualset3
135967	5	406949	5	NULL	NULL	0	NULL	hexanal contents 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significantly ( P & lt ; 0.05 ) lower values of TBARS , peroxide values , and hexanal contents were obtained for GK treated samples compared with cooked pork without antioxidant during refrigerated storage .
	manualset3
135968	6	406949	5	NULL	NULL	0	NULL	GK treated samples	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significantly ( P & lt ; 0.05 ) lower values of TBARS , peroxide values , and hexanal contents were obtained for GK treated samples compared with cooked pork without antioxidant during refrigerated storage .
	manualset3
135969	7	406949	5	NULL	NULL	0	NULL	cooked pork	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Significantly ( P & lt ; 0.05 ) lower values of TBARS , peroxide values , and hexanal contents were obtained for GK treated samples compared with cooked pork without antioxidant during refrigerated storage .
	manualset3
135970	8	406949	5	NULL	NULL	0	NULL	antioxidant 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Significantly ( P & lt ; 0.05 ) lower values of TBARS , peroxide values , and hexanal contents were obtained for GK treated samples compared with cooked pork without antioxidant during refrigerated storage .
	manualset3
135971	9	406949	5	NULL	NULL	0	NULL	refrigerated storage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Significantly ( P & lt ; 0.05 ) lower values of TBARS , peroxide values , and hexanal contents were obtained for GK treated samples compared with cooked pork without antioxidant during refrigerated storage .
	manualset3
135972	1	406950	5	NULL	NULL	0	NULL	pTF 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Significantly , we demonstrated that the pTF interacts with the promoters of the deregulated HBx target genes and that deregulation by HBx of these HBx target genes carrying the pTF consensus sequences can be reversed using pTF small interfering RNAs .
	manualset3
135973	2	406950	5	NULL	NULL	0	NULL	promoters 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Significantly , we demonstrated that the pTF interacts with the promoters of the deregulated HBx target genes and that deregulation by HBx of these HBx target genes carrying the pTF consensus sequences can be reversed using pTF small interfering RNAs .
	manualset3
135974	3	406950	5	NULL	NULL	0	NULL	HBx target genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Significantly , we demonstrated that the pTF interacts with the promoters of the deregulated HBx target genes and that deregulation by HBx of these HBx target genes carrying the pTF consensus sequences can be reversed using pTF small interfering RNAs .
	manualset3
135975	4	406950	5	NULL	NULL	0	NULL	deregulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Significantly , we demonstrated that the pTF interacts with the promoters of the deregulated HBx target genes and that deregulation by HBx of these HBx target genes carrying the pTF consensus sequences can be reversed using pTF small interfering RNAs .
	manualset3
135976	5	406950	5	NULL	NULL	0	NULL	HBx 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Significantly , we demonstrated that the pTF interacts with the promoters of the deregulated HBx target genes and that deregulation by HBx of these HBx target genes carrying the pTF consensus sequences can be reversed using pTF small interfering RNAs .
	manualset3
135977	6	406950	5	NULL	NULL	0	NULL	 HBx target genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Significantly , we demonstrated that the pTF interacts with the promoters of the deregulated HBx target genes and that deregulation by HBx of these HBx target genes carrying the pTF consensus sequences can be reversed using pTF small interfering RNAs .
	manualset3
135978	7	406950	5	NULL	NULL	0	NULL	pTF consensus sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Significantly , we demonstrated that the pTF interacts with the promoters of the deregulated HBx target genes and that deregulation by HBx of these HBx target genes carrying the pTF consensus sequences can be reversed using pTF small interfering RNAs .
	manualset3
135979	8	406950	5	NULL	NULL	0	NULL	pTF small interfering RNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Significantly , we demonstrated that the pTF interacts with the promoters of the deregulated HBx target genes and that deregulation by HBx of these HBx target genes carrying the pTF consensus sequences can be reversed using pTF small interfering RNAs .
	manualset3
135980	1	406951	5	NULL	NULL	0	NULL	 increased levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significantly increased levels of EGF and EGF-R were present in neoplastic samples compared to surrounding mucosa .
	manualset3
135981	2	406951	5	NULL	NULL	0	NULL	EGF 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Significantly increased levels of EGF and EGF-R were present in neoplastic samples compared to surrounding mucosa .
	manualset3
135982	3	406951	5	NULL	NULL	0	NULL	EGF-R 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Significantly increased levels of EGF and EGF-R were present in neoplastic samples compared to surrounding mucosa .
	manualset3
135983	4	406951	5	NULL	NULL	0	NULL	neoplastic samples	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significantly increased levels of EGF and EGF-R were present in neoplastic samples compared to surrounding mucosa .
	manualset3
135984	5	406951	5	NULL	NULL	0	NULL	surrounding mucosa	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Significantly increased levels of EGF and EGF-R were present in neoplastic samples compared to surrounding mucosa .
	manualset3
135985	1	406952	5	NULL	NULL	0	NULL	Signs 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Signs of diverticulitis may mask the presence of cancer , and the diagnosis of associated lesions is sometimes difficult .
	manualset3
135986	2	406952	5	NULL	NULL	0	NULL	diverticulitis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Signs of diverticulitis may mask the presence of cancer , and the diagnosis of associated lesions is sometimes difficult .
	manualset3
135987	3	406952	5	NULL	NULL	0	NULL	mask 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Signs of diverticulitis may mask the presence of cancer , and the diagnosis of associated lesions is sometimes difficult .
	manualset3
135988	4	406952	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Signs of diverticulitis may mask the presence of cancer , and the diagnosis of associated lesions is sometimes difficult .
	manualset3
135989	5	406952	5	NULL	NULL	0	NULL	cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Signs of diverticulitis may mask the presence of cancer , and the diagnosis of associated lesions is sometimes difficult .
	manualset3
135990	6	406952	5	NULL	NULL	0	NULL	diagnosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Signs of diverticulitis may mask the presence of cancer , and the diagnosis of associated lesions is sometimes difficult .
	manualset3
135991	7	406952	5	NULL	NULL	0	NULL	associated lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Signs of diverticulitis may mask the presence of cancer , and the diagnosis of associated lesions is sometimes difficult .
	manualset3
135992	1	406953	5	NULL	NULL	0	NULL	finding 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel finding of this study lies in the sensitivity of BEI to detect AN , presumably because of its combination of parameters that measure reductions in both sympathetic control of vasomotion and parasympathetic control of heart rate .
	manualset3
135993	2	406953	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel finding of this study lies in the sensitivity of BEI to detect AN , presumably because of its combination of parameters that measure reductions in both sympathetic control of vasomotion and parasympathetic control of heart rate .
	manualset3
135994	3	406953	5	NULL	NULL	0	NULL	sensitivity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel finding of this study lies in the sensitivity of BEI to detect AN , presumably because of its combination of parameters that measure reductions in both sympathetic control of vasomotion and parasympathetic control of heart rate .
	manualset3
135995	4	406953	5	NULL	NULL	0	NULL	BEI 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel finding of this study lies in the sensitivity of BEI to detect AN , presumably because of its combination of parameters that measure reductions in both sympathetic control of vasomotion and parasympathetic control of heart rate .
	manualset3
135996	5	406953	5	NULL	NULL	0	NULL	AN 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel finding of this study lies in the sensitivity of BEI to detect AN , presumably because of its combination of parameters that measure reductions in both sympathetic control of vasomotion and parasympathetic control of heart rate .
	manualset3
135997	6	406953	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel finding of this study lies in the sensitivity of BEI to detect AN , presumably because of its combination of parameters that measure reductions in both sympathetic control of vasomotion and parasympathetic control of heart rate .
	manualset3
135998	7	406953	5	NULL	NULL	0	NULL	parameters 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel finding of this study lies in the sensitivity of BEI to detect AN , presumably because of its combination of parameters that measure reductions in both sympathetic control of vasomotion and parasympathetic control of heart rate .
	manualset3
135999	8	406953	5	NULL	NULL	0	NULL	reductions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel finding of this study lies in the sensitivity of BEI to detect AN , presumably because of its combination of parameters that measure reductions in both sympathetic control of vasomotion and parasympathetic control of heart rate .
	manualset3
136000	9	406953	5	NULL	NULL	0	NULL	sympathetic control 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel finding of this study lies in the sensitivity of BEI to detect AN , presumably because of its combination of parameters that measure reductions in both sympathetic control of vasomotion and parasympathetic control of heart rate .
	manualset3
136001	10	406953	5	NULL	NULL	0	NULL	vasomotion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel finding of this study lies in the sensitivity of BEI to detect AN , presumably because of its combination of parameters that measure reductions in both sympathetic control of vasomotion and parasympathetic control of heart rate .
	manualset3
136002	11	406953	5	NULL	NULL	0	NULL	parasympathetic control	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel finding of this study lies in the sensitivity of BEI to detect AN , presumably because of its combination of parameters that measure reductions in both sympathetic control of vasomotion and parasympathetic control of heart rate .
	manualset3
136003	12	406953	5	NULL	NULL	0	NULL	heart rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel finding of this study lies in the sensitivity of BEI to detect AN , presumably because of its combination of parameters that measure reductions in both sympathetic control of vasomotion and parasympathetic control of heart rate .
	manualset3
136004	1	406954	5	NULL	NULL	0	NULL	Signs 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Signs of postoperative distress ( pain , nausea , drowsiness ) were evaluated after 2 and 6 h by visual analog scale scores .
	manualset3
136005	2	406954	5	NULL	NULL	0	NULL	postoperative distress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Signs of postoperative distress ( pain , nausea , drowsiness ) were evaluated after 2 and 6 h by visual analog scale scores .
	manualset3
136006	3	406954	5	NULL	NULL	0	NULL	pain 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Signs of postoperative distress ( pain , nausea , drowsiness ) were evaluated after 2 and 6 h by visual analog scale scores .
	manualset3
136007	4	406954	5	NULL	NULL	0	NULL	nausea 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Signs of postoperative distress ( pain , nausea , drowsiness ) were evaluated after 2 and 6 h by visual analog scale scores .
	manualset3
136008	5	406954	5	NULL	NULL	0	NULL	drowsiness 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Signs of postoperative distress ( pain , nausea , drowsiness ) were evaluated after 2 and 6 h by visual analog scale scores .
	manualset3
136009	6	406954	5	NULL	NULL	0	NULL	2 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Signs of postoperative distress ( pain , nausea , drowsiness ) were evaluated after 2 and 6 h by visual analog scale scores .
	manualset3
136010	7	406954	5	NULL	NULL	0	NULL	6 h 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Signs of postoperative distress ( pain , nausea , drowsiness ) were evaluated after 2 and 6 h by visual analog scale scores .
	manualset3
136011	8	406954	5	NULL	NULL	0	NULL	visual analog scale scores	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Signs of postoperative distress ( pain , nausea , drowsiness ) were evaluated after 2 and 6 h by visual analog scale scores .
	manualset3
136012	1	406955	5	NULL	NULL	0	NULL	Sigsearch 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sigsearch : a new term for post hoc unplanned search for statistically significant relationships with the intent to create publishable findings .
	manualset3
136013	2	406955	5	NULL	NULL	0	NULL	post hoc unplanned search	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sigsearch : a new term for post hoc unplanned search for statistically significant relationships with the intent to create publishable findings .
	manualset3
136014	3	406955	5	NULL	NULL	0	NULL	statistically significant relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Sigsearch : a new term for post hoc unplanned search for statistically significant relationships with the intent to create publishable findings .
	manualset3
136015	4	406955	5	NULL	NULL	0	NULL	publishable findings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sigsearch : a new term for post hoc unplanned search for statistically significant relationships with the intent to create publishable findings .
	manualset3
136016	1	406956	5	NULL	NULL	0	NULL	Silastic foam dressings	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Silastic foam dressings are indicated in cases of badly healing and infected wounds , especially caused by diabetes and arteriosclerosis .
	manualset3
136017	2	406956	5	NULL	NULL	0	NULL	cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Silastic foam dressings are indicated in cases of badly healing and infected wounds , especially caused by diabetes and arteriosclerosis .
	manualset3
136018	3	406956	5	NULL	NULL	0	NULL	badly healing and infected wounds	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Silastic foam dressings are indicated in cases of badly healing and infected wounds , especially caused by diabetes and arteriosclerosis .
	manualset3
136019	4	406956	5	NULL	NULL	0	NULL	diabetes 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Silastic foam dressings are indicated in cases of badly healing and infected wounds , especially caused by diabetes and arteriosclerosis .
	manualset3
136020	5	406956	5	NULL	NULL	0	NULL	arteriosclerosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Silastic foam dressings are indicated in cases of badly healing and infected wounds , especially caused by diabetes and arteriosclerosis .
	manualset3
136021	1	406957	5	NULL	NULL	0	NULL	Silencing 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Silencing of RGS10 by means of adenovirus-mediated transcription of a short hairpin RNA did not affect basal tau ( d ) but removed sensitivity to Iso .
	manualset3
136022	2	406957	5	NULL	NULL	0	NULL	RGS10 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Silencing of RGS10 by means of adenovirus-mediated transcription of a short hairpin RNA did not affect basal tau ( d ) but removed sensitivity to Iso .
	manualset3
136023	3	406957	5	NULL	NULL	0	NULL	adenovirus-mediated transcription 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Silencing of RGS10 by means of adenovirus-mediated transcription of a short hairpin RNA did not affect basal tau ( d ) but removed sensitivity to Iso .
	manualset3
136024	4	406957	5	NULL	NULL	0	NULL	short hairpin RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Silencing of RGS10 by means of adenovirus-mediated transcription of a short hairpin RNA did not affect basal tau ( d ) but removed sensitivity to Iso .
	manualset3
136025	5	406957	5	NULL	NULL	0	NULL	basal tau ( d )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Silencing of RGS10 by means of adenovirus-mediated transcription of a short hairpin RNA did not affect basal tau ( d ) but removed sensitivity to Iso .
	manualset3
136026	6	406957	5	NULL	NULL	0	NULL	sensitivity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Silencing of RGS10 by means of adenovirus-mediated transcription of a short hairpin RNA did not affect basal tau ( d ) but removed sensitivity to Iso .
	manualset3
136027	7	406957	5	NULL	NULL	0	NULL	Iso 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Silencing of RGS10 by means of adenovirus-mediated transcription of a short hairpin RNA did not affect basal tau ( d ) but removed sensitivity to Iso .
	manualset3
136028	1	406958	5	NULL	NULL	0	NULL	Silicone oil 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Silicone oil does appear to act as a diffusion/convection barrier to oxygen and may alter the stimulus for anterior segment neovascularization .
	manualset3
136029	2	406958	5	NULL	NULL	0	NULL	diffusion/convection barrier 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Silicone oil does appear to act as a diffusion/convection barrier to oxygen and may alter the stimulus for anterior segment neovascularization .
	manualset3
136030	3	406958	5	NULL	NULL	0	NULL	oxygen 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Silicone oil does appear to act as a diffusion/convection barrier to oxygen and may alter the stimulus for anterior segment neovascularization .
	manualset3
136031	4	406958	5	NULL	NULL	0	NULL	stimulus 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Silicone oil does appear to act as a diffusion/convection barrier to oxygen and may alter the stimulus for anterior segment neovascularization .
	manualset3
136032	5	406958	5	NULL	NULL	0	NULL	anterior segment neovascularization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Silicone oil does appear to act as a diffusion/convection barrier to oxygen and may alter the stimulus for anterior segment neovascularization .
	manualset3
136033	1	406959	5	NULL	NULL	0	NULL	Silk I	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Silk I and silk II are the structures of silk fibroin before and after spinning , respectively .
	manualset3
136034	2	406959	5	NULL	NULL	0	NULL	silk II	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Silk I and silk II are the structures of silk fibroin before and after spinning , respectively .
	manualset3
136035	3	406959	5	NULL	NULL	0	NULL	structures 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Silk I and silk II are the structures of silk fibroin before and after spinning , respectively .
	manualset3
136036	4	406959	5	NULL	NULL	0	NULL	silk fibroin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Silk I and silk II are the structures of silk fibroin before and after spinning , respectively .
	manualset3
136037	5	406959	5	NULL	NULL	0	NULL	spinning 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Silk I and silk II are the structures of silk fibroin before and after spinning , respectively .
	manualset3
136038	1	406960	5	NULL	NULL	0	NULL	Silver allergy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Silver allergy does occur but the extent of the problem is not known .
	manualset3
136039	2	406960	5	NULL	NULL	0	NULL	extent 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Silver allergy does occur but the extent of the problem is not known .
	manualset3
136040	3	406960	5	NULL	NULL	0	NULL	problem 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Silver allergy does occur but the extent of the problem is not known .
	manualset3
136041	1	406961	5	NULL	NULL	0	NULL	Simian virus 40-transformed fibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Simian virus 40-transformed fibroblasts also produced the SF antigen , as shown by radioimmunoassay or immunodiffusion tests , but it was not retained by the surface of these cells .
	manualset3
136042	2	406961	5	NULL	NULL	0	NULL	SF antigen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Simian virus 40-transformed fibroblasts also produced the SF antigen , as shown by radioimmunoassay or immunodiffusion tests , but it was not retained by the surface of these cells .
	manualset3
136043	3	406961	5	NULL	NULL	0	NULL	radioimmunoassay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Simian virus 40-transformed fibroblasts also produced the SF antigen , as shown by radioimmunoassay or immunodiffusion tests , but it was not retained by the surface of these cells .
	manualset3
136044	4	406961	5	NULL	NULL	0	NULL	immunodiffusion tests	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Simian virus 40-transformed fibroblasts also produced the SF antigen , as shown by radioimmunoassay or immunodiffusion tests , but it was not retained by the surface of these cells .
	manualset3
136045	5	406961	5	NULL	NULL	0	NULL	surface 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Simian virus 40-transformed fibroblasts also produced the SF antigen , as shown by radioimmunoassay or immunodiffusion tests , but it was not retained by the surface of these cells .
	manualset3
136046	6	406961	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Simian virus 40-transformed fibroblasts also produced the SF antigen , as shown by radioimmunoassay or immunodiffusion tests , but it was not retained by the surface of these cells .
	manualset3
136047	1	406962	5	NULL	NULL	0	NULL	prominent effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar , but slightly less prominent effects were observed when aspartic acid was added instead of glutamic acid .
	manualset3
136048	2	406962	5	NULL	NULL	0	NULL	aspartic acid 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar , but slightly less prominent effects were observed when aspartic acid was added instead of glutamic acid .
	manualset3
136049	3	406962	5	NULL	NULL	0	NULL	glutamic acid	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar , but slightly less prominent effects were observed when aspartic acid was added instead of glutamic acid .
	manualset3
136050	1	406963	5	NULL	NULL	NULL	NULL	 Central nervous system relapse 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Central nervous system relapse with multiple brain masses in an acute promyelocytic leukemia patient treated with all-trans retinoic acid ) .
	manualset3
136051	2	406963	5	NULL	NULL	0	NULL	multiple brain masses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Central nervous system relapse with multiple brain masses in an acute promyelocytic leukemia patient treated with all-trans retinoic acid ) .
	manualset3
136052	3	406963	5	NULL	NULL	0	NULL	acute promyelocytic leukemia patient	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Central nervous system relapse with multiple brain masses in an acute promyelocytic leukemia patient treated with all-trans retinoic acid ) .
	manualset3
136053	4	406963	5	NULL	NULL	0	NULL	all-trans retinoic acid	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Central nervous system relapse with multiple brain masses in an acute promyelocytic leukemia patient treated with all-trans retinoic acid ) .
	manualset3
136054	1	406964	5	NULL	NULL	0	NULL	novel fungus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel fungus with high nitrile hydrolase was newly isolated from soil samples and identified as Fusarium oxysporum H3 through 18S ribosomal DNA , 28S ribosomal DNA , and the internal transcribed spacer sequence analysis , together with morphology characteristics .
	manualset3
136055	2	406964	5	NULL	NULL	0	NULL	high nitrile hydrolase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel fungus with high nitrile hydrolase was newly isolated from soil samples and identified as Fusarium oxysporum H3 through 18S ribosomal DNA , 28S ribosomal DNA , and the internal transcribed spacer sequence analysis , together with morphology characteristics .
	manualset3
136056	3	406964	5	NULL	NULL	0	NULL	soil samples	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel fungus with high nitrile hydrolase was newly isolated from soil samples and identified as Fusarium oxysporum H3 through 18S ribosomal DNA , 28S ribosomal DNA , and the internal transcribed spacer sequence analysis , together with morphology characteristics .
	manualset3
136057	4	406964	5	NULL	NULL	0	NULL	Fusarium oxysporum H3	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel fungus with high nitrile hydrolase was newly isolated from soil samples and identified as Fusarium oxysporum H3 through 18S ribosomal DNA , 28S ribosomal DNA , and the internal transcribed spacer sequence analysis , together with morphology characteristics .
	manualset3
136058	5	406964	5	NULL	NULL	0	NULL	18S ribosomal DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel fungus with high nitrile hydrolase was newly isolated from soil samples and identified as Fusarium oxysporum H3 through 18S ribosomal DNA , 28S ribosomal DNA , and the internal transcribed spacer sequence analysis , together with morphology characteristics .
	manualset3
136059	6	406964	5	NULL	NULL	0	NULL	28S ribosomal DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel fungus with high nitrile hydrolase was newly isolated from soil samples and identified as Fusarium oxysporum H3 through 18S ribosomal DNA , 28S ribosomal DNA , and the internal transcribed spacer sequence analysis , together with morphology characteristics .
	manualset3
136060	7	406964	5	NULL	NULL	0	NULL	internal transcribed spacer sequence analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel fungus with high nitrile hydrolase was newly isolated from soil samples and identified as Fusarium oxysporum H3 through 18S ribosomal DNA , 28S ribosomal DNA , and the internal transcribed spacer sequence analysis , together with morphology characteristics .
	manualset3
136061	8	406964	5	NULL	NULL	0	NULL	morphology characteristics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel fungus with high nitrile hydrolase was newly isolated from soil samples and identified as Fusarium oxysporum H3 through 18S ribosomal DNA , 28S ribosomal DNA , and the internal transcribed spacer sequence analysis , together with morphology characteristics .
	manualset3
136062	1	406965	5	NULL	NULL	0	NULL	analyses 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar analyses of the colostomy contents of subjects revealed a total menaquinone content of 8.85 micrograms/g dry weight .
	manualset3
136063	2	406965	5	NULL	NULL	0	NULL	colostomy contents 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar analyses of the colostomy contents of subjects revealed a total menaquinone content of 8.85 micrograms/g dry weight .
	manualset3
136064	3	406965	5	NULL	NULL	0	NULL	subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar analyses of the colostomy contents of subjects revealed a total menaquinone content of 8.85 micrograms/g dry weight .
	manualset3
136065	4	406965	5	NULL	NULL	0	NULL	total menaquinone content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar analyses of the colostomy contents of subjects revealed a total menaquinone content of 8.85 micrograms/g dry weight .
	manualset3
136066	5	406965	5	NULL	NULL	0	NULL	8.85 micrograms/g dry weight	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar analyses of the colostomy contents of subjects revealed a total menaquinone content of 8.85 micrograms/g dry weight .
	manualset3
136067	1	406966	5	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar binding of OC 133 was observed with three of the four ovarian tumor cell lines .
	manualset3
136068	2	406966	5	NULL	NULL	0	NULL	OC 133 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar binding of OC 133 was observed with three of the four ovarian tumor cell lines .
	manualset3
136069	3	406966	5	NULL	NULL	0	NULL	three of the four 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar binding of OC 133 was observed with three of the four ovarian tumor cell lines .
	manualset3
136070	4	406966	5	NULL	NULL	0	NULL	ovarian tumor cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar binding of OC 133 was observed with three of the four ovarian tumor cell lines .
	manualset3
136071	1	406967	5	NULL	NULL	0	NULL	delayed inward currents	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar delayed inward currents were activated by both caged compounds but only NPE-caged cGMP evoked rapidly activating currents .
	manualset3
136072	2	406967	5	NULL	NULL	0	NULL	caged compounds	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar delayed inward currents were activated by both caged compounds but only NPE-caged cGMP evoked rapidly activating currents .
	manualset3
136073	3	406967	5	NULL	NULL	0	NULL	NPE-caged cGMP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar delayed inward currents were activated by both caged compounds but only NPE-caged cGMP evoked rapidly activating currents .
	manualset3
136074	4	406967	5	NULL	NULL	0	NULL	rapidly activating currents	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar delayed inward currents were activated by both caged compounds but only NPE-caged cGMP evoked rapidly activating currents .
	manualset3
136075	1	406968	5	NULL	NULL	0	NULL	granulomas 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar granulomas in the spleen and lymph nodes as well as in other tissues have been described in polyarteritis nodosa .
	manualset3
136076	2	406968	5	NULL	NULL	0	NULL	spleen 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar granulomas in the spleen and lymph nodes as well as in other tissues have been described in polyarteritis nodosa .
	manualset3
136077	3	406968	5	NULL	NULL	0	NULL	lymph nodes 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar granulomas in the spleen and lymph nodes as well as in other tissues have been described in polyarteritis nodosa .
	manualset3
136078	4	406968	5	NULL	NULL	0	NULL	tissues 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar granulomas in the spleen and lymph nodes as well as in other tissues have been described in polyarteritis nodosa .
	manualset3
136079	5	406968	5	NULL	NULL	0	NULL	polyarteritis nodosa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar granulomas in the spleen and lymph nodes as well as in other tissues have been described in polyarteritis nodosa .
	manualset3
136080	1	406969	5	NULL	NULL	0	NULL	pulse-chase experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar pulse-chase experiments followed by immunoprecipitation using affinity purified antiserum have been used to investigate the addition of the cross-reacting determinant .
	manualset3
136081	2	406969	5	NULL	NULL	0	NULL	immunoprecipitation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar pulse-chase experiments followed by immunoprecipitation using affinity purified antiserum have been used to investigate the addition of the cross-reacting determinant .
	manualset3
136082	3	406969	5	NULL	NULL	0	NULL	affinity purified antiserum	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar pulse-chase experiments followed by immunoprecipitation using affinity purified antiserum have been used to investigate the addition of the cross-reacting determinant .
	manualset3
136083	4	406969	5	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar pulse-chase experiments followed by immunoprecipitation using affinity purified antiserum have been used to investigate the addition of the cross-reacting determinant .
	manualset3
136084	5	406969	5	NULL	NULL	0	NULL	cross-reacting determinant	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar pulse-chase experiments followed by immunoprecipitation using affinity purified antiserum have been used to investigate the addition of the cross-reacting determinant .
	manualset3
136085	1	406970	5	NULL	NULL	0	NULL	responses 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar responses to NE were seen after additional priming with P at the same time as EB .
	manualset3
136086	2	406970	5	NULL	NULL	0	NULL	NE 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar responses to NE were seen after additional priming with P at the same time as EB .
	manualset3
136087	3	406970	5	NULL	NULL	0	NULL	priming 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar responses to NE were seen after additional priming with P at the same time as EB .
	manualset3
136088	4	406970	5	NULL	NULL	0	NULL	P	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar responses to NE were seen after additional priming with P at the same time as EB .
	manualset3
136089	5	406970	5	NULL	NULL	NULL	NULL	EB	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Similar responses to NE were seen after additional priming with P at the same time as EB .
	manualset3
136090	1	406971	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar results were also found under additive ( OR = 1.57 , 95 % CI : 1.10-2 .23 ) and dominant ( OR = 1.40 , 95 % CI : 1.06-1 .85 ) genetic models .
	manualset3
136091	2	406971	5	NULL	NULL	0	NULL	 OR = 1.57 , 95 % CI : 1.10-2 .23 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar results were also found under additive ( OR = 1.57 , 95 % CI : 1.10-2 .23 ) and dominant ( OR = 1.40 , 95 % CI : 1.06-1 .85 ) genetic models .
	manualset3
136092	3	406971	5	NULL	NULL	0	NULL	additive genetic models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar results were also found under additive ( OR = 1.57 , 95 % CI : 1.10-2 .23 ) and dominant ( OR = 1.40 , 95 % CI : 1.06-1 .85 ) genetic models .
	manualset3
136093	4	406971	5	NULL	NULL	0	NULL	dominant genetic models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar results were also found under additive ( OR = 1.57 , 95 % CI : 1.10-2 .23 ) and dominant ( OR = 1.40 , 95 % CI : 1.06-1 .85 ) genetic models .
	manualset3
136094	5	406971	5	NULL	NULL	0	NULL	OR = 1.40 , 95 % CI : 1.06-1 .85	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar results were also found under additive ( OR = 1.57 , 95 % CI : 1.10-2 .23 ) and dominant ( OR = 1.40 , 95 % CI : 1.06-1 .85 ) genetic models .
	manualset3
136095	1	406972	5	NULL	NULL	0	NULL	novel immune algorithm	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel immune algorithm for resolution and quantitative determination of the components in overlapping chromatograms was proposed by imitating biological immune systems .
	manualset3
136096	2	406972	5	NULL	NULL	0	NULL	resolution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel immune algorithm for resolution and quantitative determination of the components in overlapping chromatograms was proposed by imitating biological immune systems .
	manualset3
136097	3	406972	5	NULL	NULL	0	NULL	quantitative determination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel immune algorithm for resolution and quantitative determination of the components in overlapping chromatograms was proposed by imitating biological immune systems .
	manualset3
136098	4	406972	5	NULL	NULL	0	NULL	components 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel immune algorithm for resolution and quantitative determination of the components in overlapping chromatograms was proposed by imitating biological immune systems .
	manualset3
136099	5	406972	5	NULL	NULL	0	NULL	overlapping chromatograms	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel immune algorithm for resolution and quantitative determination of the components in overlapping chromatograms was proposed by imitating biological immune systems .
	manualset3
136100	6	406972	5	NULL	NULL	0	NULL	biological immune systems	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel immune algorithm for resolution and quantitative determination of the components in overlapping chromatograms was proposed by imitating biological immune systems .
	manualset3
136101	1	406973	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar results were observed with the phosphodiesterase inhibitor milrinone .
	manualset3
136102	2	406973	5	NULL	NULL	0	NULL	phosphodiesterase inhibitor milrinone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar results were observed with the phosphodiesterase inhibitor milrinone .
	manualset3
136103	1	406974	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar results were obtained by measuring N2O and isoflurane concentrations at the ventilator zone and in urine .
	manualset3
136104	2	406974	5	NULL	NULL	0	NULL	N2O concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar results were obtained by measuring N2O and isoflurane concentrations at the ventilator zone and in urine .
	manualset3
136105	3	406974	5	NULL	NULL	0	NULL	isoflurane concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar results were obtained by measuring N2O and isoflurane concentrations at the ventilator zone and in urine .
	manualset3
136106	4	406974	5	NULL	NULL	0	NULL	ventilator zone	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar results were obtained by measuring N2O and isoflurane concentrations at the ventilator zone and in urine .
	manualset3
136107	5	406974	5	NULL	NULL	0	NULL	urine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar results were obtained by measuring N2O and isoflurane concentrations at the ventilator zone and in urine .
	manualset3
136108	1	406975	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar results with the C. michiganensis subsp .
	manualset3
136109	2	406975	5	NULL	NULL	0	NULL	C. michiganensis subsp	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar results with the C. michiganensis subsp .
	manualset3
136110	1	406976	5	NULL	NULL	0	NULL	HCMV 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to HCMV , CyCMV does not produce the RhCMV-specific viral homolog of cyclooxygenase-2 .
	manualset3
136111	2	406976	5	NULL	NULL	0	NULL	CyCMV 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to HCMV , CyCMV does not produce the RhCMV-specific viral homolog of cyclooxygenase-2 .
	manualset3
136112	3	406976	5	NULL	NULL	0	NULL	RhCMV-specific viral homolog of cyclooxygenase-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to HCMV , CyCMV does not produce the RhCMV-specific viral homolog of cyclooxygenase-2 .
	manualset3
136113	1	406977	5	NULL	NULL	0	NULL	mammalian sAC	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to mammalian sAC , dogfish soluble adenylyl cyclase ( dfsAC ) is activated by HCO ( 3 ) ( - ) and can be inhibited by two structurally and mechanistically distinct small molecule inhibitors .
	manualset3
136114	2	406977	5	NULL	NULL	0	NULL	dogfish soluble adenylyl cyclase ( dfsAC )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to mammalian sAC , dogfish soluble adenylyl cyclase ( dfsAC ) is activated by HCO ( 3 ) ( - ) and can be inhibited by two structurally and mechanistically distinct small molecule inhibitors .
	manualset3
136115	3	406977	5	NULL	NULL	0	NULL	HCO ( 3 ) ( - ) 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to mammalian sAC , dogfish soluble adenylyl cyclase ( dfsAC ) is activated by HCO ( 3 ) ( - ) and can be inhibited by two structurally and mechanistically distinct small molecule inhibitors .
	manualset3
136116	4	406977	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to mammalian sAC , dogfish soluble adenylyl cyclase ( dfsAC ) is activated by HCO ( 3 ) ( - ) and can be inhibited by two structurally and mechanistically distinct small molecule inhibitors .
	manualset3
136117	5	406977	5	NULL	NULL	0	NULL	small molecule inhibitors	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to mammalian sAC , dogfish soluble adenylyl cyclase ( dfsAC ) is activated by HCO ( 3 ) ( - ) and can be inhibited by two structurally and mechanistically distinct small molecule inhibitors .
	manualset3
136118	1	406978	5	NULL	NULL	0	NULL	blood purification therapies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to other blood purification therapies , therapeutic intensity , molecular weight , and half life are crucial factors for solute removal .
	manualset3
136119	2	406978	5	NULL	NULL	0	NULL	therapeutic intensity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to other blood purification therapies , therapeutic intensity , molecular weight , and half life are crucial factors for solute removal .
	manualset3
136120	3	406978	5	NULL	NULL	0	NULL	molecular weight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to other blood purification therapies , therapeutic intensity , molecular weight , and half life are crucial factors for solute removal .
	manualset3
136121	4	406978	5	NULL	NULL	0	NULL	half life	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to other blood purification therapies , therapeutic intensity , molecular weight , and half life are crucial factors for solute removal .
	manualset3
136122	5	406978	5	NULL	NULL	0	NULL	crucial factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to other blood purification therapies , therapeutic intensity , molecular weight , and half life are crucial factors for solute removal .
	manualset3
136123	6	406978	5	NULL	NULL	0	NULL	solute removal	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to other blood purification therapies , therapeutic intensity , molecular weight , and half life are crucial factors for solute removal .
	manualset3
136124	1	406979	5	NULL	NULL	0	NULL	peroxidases 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to other peroxidases the distal histidine in KatGs forms a hydrogen bond with an adjacent conserved asparagine .
	manualset3
136125	2	406979	5	NULL	NULL	0	NULL	histidine 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to other peroxidases the distal histidine in KatGs forms a hydrogen bond with an adjacent conserved asparagine .
	manualset3
136126	3	406979	5	NULL	NULL	0	NULL	KatGs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to other peroxidases the distal histidine in KatGs forms a hydrogen bond with an adjacent conserved asparagine .
	manualset3
136127	4	406979	5	NULL	NULL	0	NULL	hydrogen bond	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to other peroxidases the distal histidine in KatGs forms a hydrogen bond with an adjacent conserved asparagine .
	manualset3
136128	5	406979	5	NULL	NULL	0	NULL	asparagine 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to other peroxidases the distal histidine in KatGs forms a hydrogen bond with an adjacent conserved asparagine .
	manualset3
136129	1	406980	5	NULL	NULL	0	NULL	fentanyl derivatives 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to several other fentanyl derivatives with clinical potential , OHM3507 had the highest affinity ( IC50 = 10 nM ) for mu ( ( 3H ) D-Ala2 , N-Me-Phe4 , Gly5-OH-labeled ) receptors with 6 - and 176-fold lower affinity for delta ( ( 3H ) D-Pen2-D-Pen5-labeled ) , and kappa ( ( 3H ) ethylketocyclazocine-labeled ) receptors , respectively .
	manualset3
136130	2	406980	5	NULL	NULL	0	NULL	clinical potential	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to several other fentanyl derivatives with clinical potential , OHM3507 had the highest affinity ( IC50 = 10 nM ) for mu ( ( 3H ) D-Ala2 , N-Me-Phe4 , Gly5-OH-labeled ) receptors with 6 - and 176-fold lower affinity for delta ( ( 3H ) D-Pen2-D-Pen5-labeled ) , and kappa ( ( 3H ) ethylketocyclazocine-labeled ) receptors , respectively .
	manualset3
136131	3	406980	5	NULL	NULL	0	NULL	OHM3507 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to several other fentanyl derivatives with clinical potential , OHM3507 had the highest affinity ( IC50 = 10 nM ) for mu ( ( 3H ) D-Ala2 , N-Me-Phe4 , Gly5-OH-labeled ) receptors with 6 - and 176-fold lower affinity for delta ( ( 3H ) D-Pen2-D-Pen5-labeled ) , and kappa ( ( 3H ) ethylketocyclazocine-labeled ) receptors , respectively .
	manualset3
136132	4	406980	5	NULL	NULL	0	NULL	highest affinity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to several other fentanyl derivatives with clinical potential , OHM3507 had the highest affinity ( IC50 = 10 nM ) for mu ( ( 3H ) D-Ala2 , N-Me-Phe4 , Gly5-OH-labeled ) receptors with 6 - and 176-fold lower affinity for delta ( ( 3H ) D-Pen2-D-Pen5-labeled ) , and kappa ( ( 3H ) ethylketocyclazocine-labeled ) receptors , respectively .
	manualset3
136133	5	406980	5	NULL	NULL	0	NULL	IC50 = 10 nM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to several other fentanyl derivatives with clinical potential , OHM3507 had the highest affinity ( IC50 = 10 nM ) for mu ( ( 3H ) D-Ala2 , N-Me-Phe4 , Gly5-OH-labeled ) receptors with 6 - and 176-fold lower affinity for delta ( ( 3H ) D-Pen2-D-Pen5-labeled ) , and kappa ( ( 3H ) ethylketocyclazocine-labeled ) receptors , respectively .
	manualset3
136134	6	406980	5	NULL	NULL	0	NULL	mu ( ( 3H ) D-Ala2 , N-Me-Phe4 , Gly5-OH-labeled ) receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to several other fentanyl derivatives with clinical potential , OHM3507 had the highest affinity ( IC50 = 10 nM ) for mu ( ( 3H ) D-Ala2 , N-Me-Phe4 , Gly5-OH-labeled ) receptors with 6 - and 176-fold lower affinity for delta ( ( 3H ) D-Pen2-D-Pen5-labeled ) , and kappa ( ( 3H ) ethylketocyclazocine-labeled ) receptors , respectively .
	manualset3
136135	7	406980	5	NULL	NULL	0	NULL	6 -fold	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to several other fentanyl derivatives with clinical potential , OHM3507 had the highest affinity ( IC50 = 10 nM ) for mu ( ( 3H ) D-Ala2 , N-Me-Phe4 , Gly5-OH-labeled ) receptors with 6 - and 176-fold lower affinity for delta ( ( 3H ) D-Pen2-D-Pen5-labeled ) , and kappa ( ( 3H ) ethylketocyclazocine-labeled ) receptors , respectively .
	manualset3
136136	8	406980	5	NULL	NULL	0	NULL	affinity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to several other fentanyl derivatives with clinical potential , OHM3507 had the highest affinity ( IC50 = 10 nM ) for mu ( ( 3H ) D-Ala2 , N-Me-Phe4 , Gly5-OH-labeled ) receptors with 6 - and 176-fold lower affinity for delta ( ( 3H ) D-Pen2-D-Pen5-labeled ) , and kappa ( ( 3H ) ethylketocyclazocine-labeled ) receptors , respectively .
	manualset3
136137	9	406980	5	NULL	NULL	0	NULL	delta ( ( 3H ) D-Pen2-D-Pen5-labeled ) receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to several other fentanyl derivatives with clinical potential , OHM3507 had the highest affinity ( IC50 = 10 nM ) for mu ( ( 3H ) D-Ala2 , N-Me-Phe4 , Gly5-OH-labeled ) receptors with 6 - and 176-fold lower affinity for delta ( ( 3H ) D-Pen2-D-Pen5-labeled ) , and kappa ( ( 3H ) ethylketocyclazocine-labeled ) receptors , respectively .
	manualset3
136138	10	406980	5	NULL	NULL	NULL	NULL	kappa ( ( 3H ) ethylketocyclazocine-labeled ) receptors 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Similar to several other fentanyl derivatives with clinical potential , OHM3507 had the highest affinity ( IC50 = 10 nM ) for mu ( ( 3H ) D-Ala2 , N-Me-Phe4 , Gly5-OH-labeled ) receptors with 6 - and 176-fold lower affinity for delta ( ( 3H ) D-Pen2-D-Pen5-labeled ) , and kappa ( ( 3H ) ethylketocyclazocine-labeled ) receptors , respectively .
	manualset3
136139	1	406981	5	NULL	NULL	0	NULL	novel laboratory screening bioassay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel laboratory screening bioassay for crop seedling allelopathy .
	manualset3
136140	2	406981	5	NULL	NULL	0	NULL	crop seedling allelopathy 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel laboratory screening bioassay for crop seedling allelopathy .
	manualset3
136141	1	406982	5	NULL	NULL	0	NULL	CYP3A4 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to that observed earlier with CYP3A4 , increasing hydrostatic pressure does not cause either a complete dissociation of the substrate complexes or a displacement of the spin equilibrium toward the low-spin state .
	manualset3
136142	2	406982	5	NULL	NULL	0	NULL	hydrostatic pressure 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to that observed earlier with CYP3A4 , increasing hydrostatic pressure does not cause either a complete dissociation of the substrate complexes or a displacement of the spin equilibrium toward the low-spin state .
	manualset3
136143	3	406982	5	NULL	NULL	0	NULL	complete dissociation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to that observed earlier with CYP3A4 , increasing hydrostatic pressure does not cause either a complete dissociation of the substrate complexes or a displacement of the spin equilibrium toward the low-spin state .
	manualset3
136144	4	406982	5	NULL	NULL	0	NULL	substrate complexes 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to that observed earlier with CYP3A4 , increasing hydrostatic pressure does not cause either a complete dissociation of the substrate complexes or a displacement of the spin equilibrium toward the low-spin state .
	manualset3
136145	5	406982	5	NULL	NULL	0	NULL	displacement 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to that observed earlier with CYP3A4 , increasing hydrostatic pressure does not cause either a complete dissociation of the substrate complexes or a displacement of the spin equilibrium toward the low-spin state .
	manualset3
136146	6	406982	5	NULL	NULL	0	NULL	spin equilibrium 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to that observed earlier with CYP3A4 , increasing hydrostatic pressure does not cause either a complete dissociation of the substrate complexes or a displacement of the spin equilibrium toward the low-spin state .
	manualset3
136147	7	406982	5	NULL	NULL	0	NULL	low-spin state	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to that observed earlier with CYP3A4 , increasing hydrostatic pressure does not cause either a complete dissociation of the substrate complexes or a displacement of the spin equilibrium toward the low-spin state .
	manualset3
136148	1	406983	5	NULL	NULL	0	NULL	mouse receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to the mouse receptor , the human IL-1 receptor contains a large cytoplasmic region and an extracellular , IL-1 binding portion composed of three immunoglobulin-like domains .
	manualset3
136149	2	406983	5	NULL	NULL	0	NULL	human IL-1 receptor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to the mouse receptor , the human IL-1 receptor contains a large cytoplasmic region and an extracellular , IL-1 binding portion composed of three immunoglobulin-like domains .
	manualset3
136150	3	406983	5	NULL	NULL	0	NULL	large cytoplasmic region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to the mouse receptor , the human IL-1 receptor contains a large cytoplasmic region and an extracellular , IL-1 binding portion composed of three immunoglobulin-like domains .
	manualset3
136151	4	406983	5	NULL	NULL	0	NULL	extracellular , IL-1 binding portion	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to the mouse receptor , the human IL-1 receptor contains a large cytoplasmic region and an extracellular , IL-1 binding portion composed of three immunoglobulin-like domains .
	manualset3
136152	5	406983	5	NULL	NULL	0	NULL	three 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to the mouse receptor , the human IL-1 receptor contains a large cytoplasmic region and an extracellular , IL-1 binding portion composed of three immunoglobulin-like domains .
	manualset3
136153	6	406983	5	NULL	NULL	0	NULL	immunoglobulin-like domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to the mouse receptor , the human IL-1 receptor contains a large cytoplasmic region and an extracellular , IL-1 binding portion composed of three immunoglobulin-like domains .
	manualset3
136154	1	406984	5	NULL	NULL	0	NULL	SPases 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to the other SPases , SpsB undergoes self-cleavage and , although the catalytic serine is retained in the self-cleavage product , a very low residual enzymatic activity remained .
	manualset3
136155	2	406984	5	NULL	NULL	0	NULL	SpsB 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to the other SPases , SpsB undergoes self-cleavage and , although the catalytic serine is retained in the self-cleavage product , a very low residual enzymatic activity remained .
	manualset3
136156	3	406984	5	NULL	NULL	0	NULL	self-cleavage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to the other SPases , SpsB undergoes self-cleavage and , although the catalytic serine is retained in the self-cleavage product , a very low residual enzymatic activity remained .
	manualset3
136157	4	406984	5	NULL	NULL	0	NULL	catalytic serine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to the other SPases , SpsB undergoes self-cleavage and , although the catalytic serine is retained in the self-cleavage product , a very low residual enzymatic activity remained .
	manualset3
136158	5	406984	5	NULL	NULL	0	NULL	self-cleavage product 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to the other SPases , SpsB undergoes self-cleavage and , although the catalytic serine is retained in the self-cleavage product , a very low residual enzymatic activity remained .
	manualset3
136159	6	406984	5	NULL	NULL	0	NULL	low residual enzymatic activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar to the other SPases , SpsB undergoes self-cleavage and , although the catalytic serine is retained in the self-cleavage product , a very low residual enzymatic activity remained .
	manualset3
136160	1	406985	5	NULL	NULL	0	NULL	colicins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities between colicins F ( Y ) and Ib , similarities between the Cir and YiuR receptors , and the detected partial cross-immunity of colicin F ( Y ) and colicin Ib producers suggest a common evolutionary origin of the colicin F ( Y ) - YiuR and colicin Ib-Cir systems .
	manualset3
136161	2	406985	5	NULL	NULL	0	NULL	F ( Y )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities between colicins F ( Y ) and Ib , similarities between the Cir and YiuR receptors , and the detected partial cross-immunity of colicin F ( Y ) and colicin Ib producers suggest a common evolutionary origin of the colicin F ( Y ) - YiuR and colicin Ib-Cir systems .
	manualset3
136162	3	406985	5	NULL	NULL	0	NULL	Ib	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities between colicins F ( Y ) and Ib , similarities between the Cir and YiuR receptors , and the detected partial cross-immunity of colicin F ( Y ) and colicin Ib producers suggest a common evolutionary origin of the colicin F ( Y ) - YiuR and colicin Ib-Cir systems .
	manualset3
136163	4	406985	5	NULL	NULL	0	NULL	Cir receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities between colicins F ( Y ) and Ib , similarities between the Cir and YiuR receptors , and the detected partial cross-immunity of colicin F ( Y ) and colicin Ib producers suggest a common evolutionary origin of the colicin F ( Y ) - YiuR and colicin Ib-Cir systems .
	manualset3
136164	5	406985	5	NULL	NULL	0	NULL	YiuR receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities between colicins F ( Y ) and Ib , similarities between the Cir and YiuR receptors , and the detected partial cross-immunity of colicin F ( Y ) and colicin Ib producers suggest a common evolutionary origin of the colicin F ( Y ) - YiuR and colicin Ib-Cir systems .
	manualset3
136165	6	406985	5	NULL	NULL	0	NULL	partial cross-immunity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities between colicins F ( Y ) and Ib , similarities between the Cir and YiuR receptors , and the detected partial cross-immunity of colicin F ( Y ) and colicin Ib producers suggest a common evolutionary origin of the colicin F ( Y ) - YiuR and colicin Ib-Cir systems .
	manualset3
136166	7	406985	5	NULL	NULL	NULL	NULL	colicin F ( Y ) producer	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Similarities between colicins F ( Y ) and Ib , similarities between the Cir and YiuR receptors , and the detected partial cross-immunity of colicin F ( Y ) and colicin Ib producers suggest a common evolutionary origin of the colicin F ( Y ) - YiuR and colicin Ib-Cir systems .
	manualset3
136167	8	406985	5	NULL	NULL	NULL	NULL	colicin Ib producer	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Similarities between colicins F ( Y ) and Ib , similarities between the Cir and YiuR receptors , and the detected partial cross-immunity of colicin F ( Y ) and colicin Ib producers suggest a common evolutionary origin of the colicin F ( Y ) - YiuR and colicin Ib-Cir systems .
	manualset3
136168	9	406985	5	NULL	NULL	0	NULL	evolutionary origin	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities between colicins F ( Y ) and Ib , similarities between the Cir and YiuR receptors , and the detected partial cross-immunity of colicin F ( Y ) and colicin Ib producers suggest a common evolutionary origin of the colicin F ( Y ) - YiuR and colicin Ib-Cir systems .
	manualset3
136169	10	406985	5	NULL	NULL	0	NULL	colicin F ( Y ) - YiuR system	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities between colicins F ( Y ) and Ib , similarities between the Cir and YiuR receptors , and the detected partial cross-immunity of colicin F ( Y ) and colicin Ib producers suggest a common evolutionary origin of the colicin F ( Y ) - YiuR and colicin Ib-Cir systems .
	manualset3
136170	11	406985	5	NULL	NULL	0	NULL	colicin Ib-Cir system	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities between colicins F ( Y ) and Ib , similarities between the Cir and YiuR receptors , and the detected partial cross-immunity of colicin F ( Y ) and colicin Ib producers suggest a common evolutionary origin of the colicin F ( Y ) - YiuR and colicin Ib-Cir systems .
	manualset3
138428	12	406985	5	NULL	NULL	0	NULL	Similarities 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities between colicins F ( Y ) and Ib , similarities between the Cir and YiuR receptors , and the detected partial cross-immunity of colicin F ( Y ) and colicin Ib producers suggest a common evolutionary origin of the colicin F ( Y ) - YiuR and colicin Ib-Cir systems .
	manualset3
138429	13	406985	5	NULL	NULL	0	NULL	similarities	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities between colicins F ( Y ) and Ib , similarities between the Cir and YiuR receptors , and the detected partial cross-immunity of colicin F ( Y ) and colicin Ib producers suggest a common evolutionary origin of the colicin F ( Y ) - YiuR and colicin Ib-Cir systems .
	manualset3
136171	1	406986	5	NULL	NULL	0	NULL	obsessive-compulsive disorder ( OCD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities between obsessive-compulsive disorder ( OCD ) and body dysmorphic disorder ( BDD ) have been described in terms of clinical presentation , comorbidity rates , treatment response profiles , and other features .
	manualset3
136172	2	406986	5	NULL	NULL	0	NULL	body dysmorphic disorder ( BDD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities between obsessive-compulsive disorder ( OCD ) and body dysmorphic disorder ( BDD ) have been described in terms of clinical presentation , comorbidity rates , treatment response profiles , and other features .
	manualset3
136173	3	406986	5	NULL	NULL	0	NULL	terms 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities between obsessive-compulsive disorder ( OCD ) and body dysmorphic disorder ( BDD ) have been described in terms of clinical presentation , comorbidity rates , treatment response profiles , and other features .
	manualset3
136174	4	406986	5	NULL	NULL	0	NULL	clinical presentation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities between obsessive-compulsive disorder ( OCD ) and body dysmorphic disorder ( BDD ) have been described in terms of clinical presentation , comorbidity rates , treatment response profiles , and other features .
	manualset3
136175	5	406986	5	NULL	NULL	0	NULL	comorbidity rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities between obsessive-compulsive disorder ( OCD ) and body dysmorphic disorder ( BDD ) have been described in terms of clinical presentation , comorbidity rates , treatment response profiles , and other features .
	manualset3
136176	6	406986	5	NULL	NULL	0	NULL	treatment response profiles	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities between obsessive-compulsive disorder ( OCD ) and body dysmorphic disorder ( BDD ) have been described in terms of clinical presentation , comorbidity rates , treatment response profiles , and other features .
	manualset3
136177	7	406986	5	NULL	NULL	0	NULL	features 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities between obsessive-compulsive disorder ( OCD ) and body dysmorphic disorder ( BDD ) have been described in terms of clinical presentation , comorbidity rates , treatment response profiles , and other features .
	manualset3
138430	8	406986	5	NULL	NULL	0	NULL	similarities 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities between obsessive-compulsive disorder ( OCD ) and body dysmorphic disorder ( BDD ) have been described in terms of clinical presentation , comorbidity rates , treatment response profiles , and other features .
	manualset3
136178	1	406987	5	NULL	NULL	0	NULL	blood parameters	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities in blood parameters observed between OVX and male rats are likely due to the suppression of ovarian hormone release after ovariectomy .
	manualset3
136179	2	406987	5	NULL	NULL	0	NULL	OVX rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities in blood parameters observed between OVX and male rats are likely due to the suppression of ovarian hormone release after ovariectomy .
	manualset3
136180	3	406987	5	NULL	NULL	0	NULL	male rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities in blood parameters observed between OVX and male rats are likely due to the suppression of ovarian hormone release after ovariectomy .
	manualset3
136181	4	406987	5	NULL	NULL	0	NULL	suppression 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities in blood parameters observed between OVX and male rats are likely due to the suppression of ovarian hormone release after ovariectomy .
	manualset3
136182	5	406987	5	NULL	NULL	0	NULL	ovarian hormone release 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities in blood parameters observed between OVX and male rats are likely due to the suppression of ovarian hormone release after ovariectomy .
	manualset3
136183	6	406987	5	NULL	NULL	0	NULL	ovariectomy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities in blood parameters observed between OVX and male rats are likely due to the suppression of ovarian hormone release after ovariectomy .
	manualset3
138431	7	406987	5	NULL	NULL	0	NULL	Similarities 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities in blood parameters observed between OVX and male rats are likely due to the suppression of ovarian hormone release after ovariectomy .
	manualset3
136184	1	406988	5	NULL	NULL	0	NULL	tooth morphology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities in tooth morphology , degree of wear , and interproximal wear facets ( IPWF ) are generally used to associate isolated teeth qualitatively .
	manualset3
136185	2	406988	5	NULL	NULL	0	NULL	degree 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities in tooth morphology , degree of wear , and interproximal wear facets ( IPWF ) are generally used to associate isolated teeth qualitatively .
	manualset3
136186	3	406988	5	NULL	NULL	0	NULL	wear 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities in tooth morphology , degree of wear , and interproximal wear facets ( IPWF ) are generally used to associate isolated teeth qualitatively .
	manualset3
136187	4	406988	5	NULL	NULL	0	NULL	interproximal wear facets ( IPWF ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities in tooth morphology , degree of wear , and interproximal wear facets ( IPWF ) are generally used to associate isolated teeth qualitatively .
	manualset3
136188	5	406988	5	NULL	NULL	0	NULL	isolated teeth	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities in tooth morphology , degree of wear , and interproximal wear facets ( IPWF ) are generally used to associate isolated teeth qualitatively .
	manualset3
138432	6	406988	5	NULL	NULL	0	NULL	Similarities 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarities in tooth morphology , degree of wear , and interproximal wear facets ( IPWF ) are generally used to associate isolated teeth qualitatively .
	manualset3
136189	1	406989	5	NULL	NULL	0	NULL	PEF	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , PEF decreased approximately 1.3 % ( p & lt ; 0.03 ) following exposure .
	manualset3
136190	2	406989	5	NULL	NULL	0	NULL	1.3 % ( p & lt ; 0.03 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , PEF decreased approximately 1.3 % ( p & lt ; 0.03 ) following exposure .
	manualset3
136191	3	406989	5	NULL	NULL	0	NULL	exposure 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , PEF decreased approximately 1.3 % ( p & lt ; 0.03 ) following exposure .
	manualset3
136192	1	406990	5	NULL	NULL	0	NULL	concrete definition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , a concrete definition for bioethics can only be attempted , more questions than answers arise .
	manualset3
136194	2	406990	5	NULL	NULL	0	NULL	bioethics 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , a concrete definition for bioethics can only be attempted , more questions than answers arise .
	manualset3
136195	3	406990	5	NULL	NULL	0	NULL	questions 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , a concrete definition for bioethics can only be attempted , more questions than answers arise .
	manualset3
136197	4	406990	5	NULL	NULL	0	NULL	answers 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , a concrete definition for bioethics can only be attempted , more questions than answers arise .
	manualset3
136200	1	406991	5	NULL	NULL	0	NULL	novel machine language genetic programming system	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel machine language genetic programming system that uses one-dimensional core memories is proposed and simulated .
	manualset3
136201	2	406991	5	NULL	NULL	0	NULL	one-dimensional core memories	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel machine language genetic programming system that uses one-dimensional core memories is proposed and simulated .
	manualset3
136203	1	406992	5	NULL	NULL	0	NULL	lower proportion	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , a lower proportion of C. albicans isolates from subjects on itraconazole therapy were susceptible to fluconazole ( 78 % ) compared to isolates from the placebo group ( 96 % ) ( P = 0.01 ) .
	manualset3
136205	2	406992	5	NULL	NULL	0	NULL	 C. albicans isolates 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , a lower proportion of C. albicans isolates from subjects on itraconazole therapy were susceptible to fluconazole ( 78 % ) compared to isolates from the placebo group ( 96 % ) ( P = 0.01 ) .
	manualset3
136207	3	406992	5	NULL	NULL	0	NULL	subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , a lower proportion of C. albicans isolates from subjects on itraconazole therapy were susceptible to fluconazole ( 78 % ) compared to isolates from the placebo group ( 96 % ) ( P = 0.01 ) .
	manualset3
136208	4	406992	5	NULL	NULL	0	NULL	itraconazole therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , a lower proportion of C. albicans isolates from subjects on itraconazole therapy were susceptible to fluconazole ( 78 % ) compared to isolates from the placebo group ( 96 % ) ( P = 0.01 ) .
	manualset3
136209	5	406992	5	NULL	NULL	0	NULL	fluconazole 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , a lower proportion of C. albicans isolates from subjects on itraconazole therapy were susceptible to fluconazole ( 78 % ) compared to isolates from the placebo group ( 96 % ) ( P = 0.01 ) .
	manualset3
136210	6	406992	5	NULL	NULL	0	NULL	78 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , a lower proportion of C. albicans isolates from subjects on itraconazole therapy were susceptible to fluconazole ( 78 % ) compared to isolates from the placebo group ( 96 % ) ( P = 0.01 ) .
	manualset3
136211	7	406992	5	NULL	NULL	0	NULL	isolates 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , a lower proportion of C. albicans isolates from subjects on itraconazole therapy were susceptible to fluconazole ( 78 % ) compared to isolates from the placebo group ( 96 % ) ( P = 0.01 ) .
	manualset3
136212	8	406992	5	NULL	NULL	0	NULL	placebo group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , a lower proportion of C. albicans isolates from subjects on itraconazole therapy were susceptible to fluconazole ( 78 % ) compared to isolates from the placebo group ( 96 % ) ( P = 0.01 ) .
	manualset3
136213	9	406992	5	NULL	NULL	0	NULL	96 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , a lower proportion of C. albicans isolates from subjects on itraconazole therapy were susceptible to fluconazole ( 78 % ) compared to isolates from the placebo group ( 96 % ) ( P = 0.01 ) .
	manualset3
136214	10	406992	5	NULL	NULL	0	NULL	 P = 0.01 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , a lower proportion of C. albicans isolates from subjects on itraconazole therapy were susceptible to fluconazole ( 78 % ) compared to isolates from the placebo group ( 96 % ) ( P = 0.01 ) .
	manualset3
136216	1	406993	5	NULL	NULL	0	NULL	competition 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , competition for ( 3H ) - granisetron binding by the 5-HT3 receptor antagonists ondansetron and tropisetron was unaffected .
	manualset3
136218	2	406993	5	NULL	NULL	0	NULL	( 3H ) - granisetron binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , competition for ( 3H ) - granisetron binding by the 5-HT3 receptor antagonists ondansetron and tropisetron was unaffected .
	manualset3
136221	3	406993	5	NULL	NULL	0	NULL	5-HT3 receptor antagonist ondansetron 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , competition for ( 3H ) - granisetron binding by the 5-HT3 receptor antagonists ondansetron and tropisetron was unaffected .
	manualset3
136222	4	406993	5	NULL	NULL	0	NULL	5-HT3 receptor antagonist tropisetron  	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , competition for ( 3H ) - granisetron binding by the 5-HT3 receptor antagonists ondansetron and tropisetron was unaffected .
	manualset3
136224	1	406994	5	NULL	NULL	0	NULL	increased SOD activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , increased SOD activity in the plasma and left ventricle was observed in SHR only .
	manualset3
136226	2	406994	5	NULL	NULL	0	NULL	plasma 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , increased SOD activity in the plasma and left ventricle was observed in SHR only .
	manualset3
136229	3	406994	5	NULL	NULL	0	NULL	left ventricle 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , increased SOD activity in the plasma and left ventricle was observed in SHR only .
	manualset3
136231	4	406994	5	NULL	NULL	0	NULL	SHR 	o												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , increased SOD activity in the plasma and left ventricle was observed in SHR only .
	manualset3
136233	1	406995	5	NULL	NULL	0	NULL	correlation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , no correlation was observed between subject age and expression of human colon arylamine N-acetyltransferase activity .
	manualset3
136235	2	406995	5	NULL	NULL	0	NULL	subject age 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , no correlation was observed between subject age and expression of human colon arylamine N-acetyltransferase activity .
	manualset3
136236	3	406995	5	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , no correlation was observed between subject age and expression of human colon arylamine N-acetyltransferase activity .
	manualset3
136238	4	406995	5	NULL	NULL	0	NULL	human colon arylamine N-acetyltransferase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , no correlation was observed between subject age and expression of human colon arylamine N-acetyltransferase activity .
	manualset3
136240	1	406996	5	NULL	NULL	0	NULL	correlation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , no significant correlation was found between ESR , CRP , anti-ds-DNA and sICAM-1 .
	manualset3
136244	2	406996	5	NULL	NULL	0	NULL	ESR 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , no significant correlation was found between ESR , CRP , anti-ds-DNA and sICAM-1 .
	manualset3
136245	3	406996	5	NULL	NULL	0	NULL	CRP 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , no significant correlation was found between ESR , CRP , anti-ds-DNA and sICAM-1 .
	manualset3
136246	4	406996	5	NULL	NULL	0	NULL	anti-ds-DNA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , no significant correlation was found between ESR , CRP , anti-ds-DNA and sICAM-1 .
	manualset3
136247	5	406996	5	NULL	NULL	0	NULL	sICAM-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , no significant correlation was found between ESR , CRP , anti-ds-DNA and sICAM-1 .
	manualset3
136248	1	406997	5	NULL	NULL	0	NULL	recent reports 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , recent reports of relationships between sleep duration and obesity have not been examined in a shift work context .
	manualset3
136249	2	406997	5	NULL	NULL	0	NULL	relationships 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , recent reports of relationships between sleep duration and obesity have not been examined in a shift work context .
	manualset3
136250	3	406997	5	NULL	NULL	0	NULL	sleep duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , recent reports of relationships between sleep duration and obesity have not been examined in a shift work context .
	manualset3
136251	4	406997	5	NULL	NULL	0	NULL	obesity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , recent reports of relationships between sleep duration and obesity have not been examined in a shift work context .
	manualset3
136252	5	406997	5	NULL	NULL	0	NULL	shift work context	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , recent reports of relationships between sleep duration and obesity have not been examined in a shift work context .
	manualset3
136253	1	406998	5	NULL	NULL	0	NULL	content 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , the content of oxytocin was lower in the neurohypophysis of rats immobilized for 24 hr but , on the contrary , increased in animals exposed to cold for 24 hr .
	manualset3
136254	2	406998	5	NULL	NULL	0	NULL	oxytocin 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , the content of oxytocin was lower in the neurohypophysis of rats immobilized for 24 hr but , on the contrary , increased in animals exposed to cold for 24 hr .
	manualset3
136255	3	406998	5	NULL	NULL	0	NULL	neurohypophysis 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , the content of oxytocin was lower in the neurohypophysis of rats immobilized for 24 hr but , on the contrary , increased in animals exposed to cold for 24 hr .
	manualset3
136256	4	406998	5	NULL	NULL	0	NULL	rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , the content of oxytocin was lower in the neurohypophysis of rats immobilized for 24 hr but , on the contrary , increased in animals exposed to cold for 24 hr .
	manualset3
136257	5	406998	5	NULL	NULL	0	NULL	24 hr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , the content of oxytocin was lower in the neurohypophysis of rats immobilized for 24 hr but , on the contrary , increased in animals exposed to cold for 24 hr .
	manualset3
136258	6	406998	5	NULL	NULL	0	NULL	animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , the content of oxytocin was lower in the neurohypophysis of rats immobilized for 24 hr but , on the contrary , increased in animals exposed to cold for 24 hr .
	manualset3
136259	7	406998	5	NULL	NULL	0	NULL	cold 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , the content of oxytocin was lower in the neurohypophysis of rats immobilized for 24 hr but , on the contrary , increased in animals exposed to cold for 24 hr .
	manualset3
136260	8	406998	5	NULL	NULL	0	NULL	24 hr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , the content of oxytocin was lower in the neurohypophysis of rats immobilized for 24 hr but , on the contrary , increased in animals exposed to cold for 24 hr .
	manualset3
136261	1	406999	5	NULL	NULL	0	NULL	extent 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , the extent of radiological bone disease was of no prognostic significance with relation to survival ( P = 0.41 ) or length of first remission ( P = 0.21 ) .
	manualset3
136262	2	406999	5	NULL	NULL	0	NULL	radiological bone disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , the extent of radiological bone disease was of no prognostic significance with relation to survival ( P = 0.41 ) or length of first remission ( P = 0.21 ) .
	manualset3
136263	3	406999	5	NULL	NULL	0	NULL	prognostic significance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , the extent of radiological bone disease was of no prognostic significance with relation to survival ( P = 0.41 ) or length of first remission ( P = 0.21 ) .
	manualset3
136264	4	406999	5	NULL	NULL	0	NULL	relation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , the extent of radiological bone disease was of no prognostic significance with relation to survival ( P = 0.41 ) or length of first remission ( P = 0.21 ) .
	manualset3
136265	5	406999	5	NULL	NULL	0	NULL	survival 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , the extent of radiological bone disease was of no prognostic significance with relation to survival ( P = 0.41 ) or length of first remission ( P = 0.21 ) .
	manualset3
136266	6	406999	5	NULL	NULL	0	NULL	P = 0.41	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , the extent of radiological bone disease was of no prognostic significance with relation to survival ( P = 0.41 ) or length of first remission ( P = 0.21 ) .
	manualset3
136267	7	406999	5	NULL	NULL	0	NULL	length 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , the extent of radiological bone disease was of no prognostic significance with relation to survival ( P = 0.41 ) or length of first remission ( P = 0.21 ) .
	manualset3
136268	8	406999	5	NULL	NULL	0	NULL	remission 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , the extent of radiological bone disease was of no prognostic significance with relation to survival ( P = 0.41 ) or length of first remission ( P = 0.21 ) .
	manualset3
136269	9	406999	5	NULL	NULL	0	NULL	P = 0.21	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , the extent of radiological bone disease was of no prognostic significance with relation to survival ( P = 0.41 ) or length of first remission ( P = 0.21 ) .
	manualset3
136271	1	407000	5	NULL	NULL	0	NULL	 liver microsomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , the liver microsomes isolated from rats pretreated with dexamethasone ( DEX-microsomes ) had a normal level of FMO activity but had enhanced rates of forming 6 beta-and 2 beta-hydroxytestosterone ( Cyp3A1 ) as well as androstenedione ( CYP3A1 ) .
	manualset3
136272	2	407000	5	NULL	NULL	0	NULL	rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , the liver microsomes isolated from rats pretreated with dexamethasone ( DEX-microsomes ) had a normal level of FMO activity but had enhanced rates of forming 6 beta-and 2 beta-hydroxytestosterone ( Cyp3A1 ) as well as androstenedione ( CYP3A1 ) .
	manualset3
136273	3	407000	5	NULL	NULL	0	NULL	dexamethasone 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , the liver microsomes isolated from rats pretreated with dexamethasone ( DEX-microsomes ) had a normal level of FMO activity but had enhanced rates of forming 6 beta-and 2 beta-hydroxytestosterone ( Cyp3A1 ) as well as androstenedione ( CYP3A1 ) .
	manualset3
136274	4	407000	5	NULL	NULL	0	NULL	DEX-microsomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , the liver microsomes isolated from rats pretreated with dexamethasone ( DEX-microsomes ) had a normal level of FMO activity but had enhanced rates of forming 6 beta-and 2 beta-hydroxytestosterone ( Cyp3A1 ) as well as androstenedione ( CYP3A1 ) .
	manualset3
136275	5	407000	5	NULL	NULL	0	NULL	normal level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , the liver microsomes isolated from rats pretreated with dexamethasone ( DEX-microsomes ) had a normal level of FMO activity but had enhanced rates of forming 6 beta-and 2 beta-hydroxytestosterone ( Cyp3A1 ) as well as androstenedione ( CYP3A1 ) .
	manualset3
136276	6	407000	5	NULL	NULL	0	NULL	FMO activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , the liver microsomes isolated from rats pretreated with dexamethasone ( DEX-microsomes ) had a normal level of FMO activity but had enhanced rates of forming 6 beta-and 2 beta-hydroxytestosterone ( Cyp3A1 ) as well as androstenedione ( CYP3A1 ) .
	manualset3
136277	7	407000	5	NULL	NULL	0	NULL	enhanced rates 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , the liver microsomes isolated from rats pretreated with dexamethasone ( DEX-microsomes ) had a normal level of FMO activity but had enhanced rates of forming 6 beta-and 2 beta-hydroxytestosterone ( Cyp3A1 ) as well as androstenedione ( CYP3A1 ) .
	manualset3
136278	8	407000	5	NULL	NULL	NULL	NULL	6 beta-and 2 beta-hydroxytestosterone ( Cyp3A1 )	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Similarly , the liver microsomes isolated from rats pretreated with dexamethasone ( DEX-microsomes ) had a normal level of FMO activity but had enhanced rates of forming 6 beta-and 2 beta-hydroxytestosterone ( Cyp3A1 ) as well as androstenedione ( CYP3A1 ) .
	manualset3
136279	9	407000	5	NULL	NULL	0	NULL	androstenedione ( CYP3A1 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , the liver microsomes isolated from rats pretreated with dexamethasone ( DEX-microsomes ) had a normal level of FMO activity but had enhanced rates of forming 6 beta-and 2 beta-hydroxytestosterone ( Cyp3A1 ) as well as androstenedione ( CYP3A1 ) .
	manualset3
136280	1	407001	5	NULL	NULL	0	NULL	novel member	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel member of the RBCC family , Trif , expressed specifically in the spermatids of mouse testis .
	manualset3
136281	2	407001	5	NULL	NULL	0	NULL	RBCC family 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel member of the RBCC family , Trif , expressed specifically in the spermatids of mouse testis .
	manualset3
136282	3	407001	5	NULL	NULL	0	NULL	Trif 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel member of the RBCC family , Trif , expressed specifically in the spermatids of mouse testis .
	manualset3
136283	4	407001	5	NULL	NULL	NULL	NULL	spermatids 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A novel member of the RBCC family , Trif , expressed specifically in the spermatids of mouse testis .
	manualset3
136284	5	407001	5	NULL	NULL	0	NULL	mouse testis 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel member of the RBCC family , Trif , expressed specifically in the spermatids of mouse testis .
	manualset3
136285	1	407002	5	NULL	NULL	0	NULL	pressure 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Simply removing pressure does n't work , but youthful drug-taking prevents hereditary mid-life failure .
	manualset3
136287	3	407002	5	NULL	NULL	0	NULL	hereditary mid-life failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Simply removing pressure does n't work , but youthful drug-taking prevents hereditary mid-life failure .
	manualset3
138433	2	407002	5	NULL	NULL	0	NULL	drug-taking	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Simply removing pressure does n't work , but youthful drug-taking prevents hereditary mid-life failure .
	manualset3
136288	1	407003	5	NULL	NULL	0	NULL	Simulation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Simulation was performed using a two-part simulation model : a volume conductor model to calculate the electrical potential distribution inside a tripolar cuff electrode and a model of a peripheral undulating human nerve fiber to simulate the fiber response to stimulation .
	manualset3
136289	2	407003	5	NULL	NULL	0	NULL	two-part simulation model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Simulation was performed using a two-part simulation model : a volume conductor model to calculate the electrical potential distribution inside a tripolar cuff electrode and a model of a peripheral undulating human nerve fiber to simulate the fiber response to stimulation .
	manualset3
136290	3	407003	5	NULL	NULL	0	NULL	volume conductor model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Simulation was performed using a two-part simulation model : a volume conductor model to calculate the electrical potential distribution inside a tripolar cuff electrode and a model of a peripheral undulating human nerve fiber to simulate the fiber response to stimulation .
	manualset3
136292	5	407003	5	NULL	NULL	0	NULL	electrical potential distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Simulation was performed using a two-part simulation model : a volume conductor model to calculate the electrical potential distribution inside a tripolar cuff electrode and a model of a peripheral undulating human nerve fiber to simulate the fiber response to stimulation .
	manualset3
136293	6	407003	5	NULL	NULL	0	NULL	tripolar cuff electrode	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Simulation was performed using a two-part simulation model : a volume conductor model to calculate the electrical potential distribution inside a tripolar cuff electrode and a model of a peripheral undulating human nerve fiber to simulate the fiber response to stimulation .
	manualset3
136294	7	407003	5	NULL	NULL	0	NULL	model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Simulation was performed using a two-part simulation model : a volume conductor model to calculate the electrical potential distribution inside a tripolar cuff electrode and a model of a peripheral undulating human nerve fiber to simulate the fiber response to stimulation .
	manualset3
136295	8	407003	5	NULL	NULL	0	NULL	peripheral undulating human nerve fiber	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Simulation was performed using a two-part simulation model : a volume conductor model to calculate the electrical potential distribution inside a tripolar cuff electrode and a model of a peripheral undulating human nerve fiber to simulate the fiber response to stimulation .
	manualset3
136296	9	407003	5	NULL	NULL	0	NULL	fiber response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Simulation was performed using a two-part simulation model : a volume conductor model to calculate the electrical potential distribution inside a tripolar cuff electrode and a model of a peripheral undulating human nerve fiber to simulate the fiber response to stimulation .
	manualset3
136297	10	407003	5	NULL	NULL	0	NULL	stimulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Simulation was performed using a two-part simulation model : a volume conductor model to calculate the electrical potential distribution inside a tripolar cuff electrode and a model of a peripheral undulating human nerve fiber to simulate the fiber response to stimulation .
	manualset3
136298	1	407004	5	NULL	NULL	0	NULL	novel method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel method for metabolic flux studies of central metabolism which is based on respirometric ( 13 ) C flux analysis , i.e. , parallel ( 13 ) C tracer studies with online CO ( 2 ) labeling measurements is applied to flux quantification of a lysine-producing mutant of Corynebacterium glutamicum .
	manualset3
136299	2	407004	5	NULL	NULL	0	NULL	metabolic flux studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel method for metabolic flux studies of central metabolism which is based on respirometric ( 13 ) C flux analysis , i.e. , parallel ( 13 ) C tracer studies with online CO ( 2 ) labeling measurements is applied to flux quantification of a lysine-producing mutant of Corynebacterium glutamicum .
	manualset3
136300	3	407004	5	NULL	NULL	0	NULL	central metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel method for metabolic flux studies of central metabolism which is based on respirometric ( 13 ) C flux analysis , i.e. , parallel ( 13 ) C tracer studies with online CO ( 2 ) labeling measurements is applied to flux quantification of a lysine-producing mutant of Corynebacterium glutamicum .
	manualset3
136301	4	407004	5	NULL	NULL	0	NULL	respirometric ( 13 ) C flux analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel method for metabolic flux studies of central metabolism which is based on respirometric ( 13 ) C flux analysis , i.e. , parallel ( 13 ) C tracer studies with online CO ( 2 ) labeling measurements is applied to flux quantification of a lysine-producing mutant of Corynebacterium glutamicum .
	manualset3
136302	5	407004	5	NULL	NULL	0	NULL	parallel ( 13 ) C tracer studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel method for metabolic flux studies of central metabolism which is based on respirometric ( 13 ) C flux analysis , i.e. , parallel ( 13 ) C tracer studies with online CO ( 2 ) labeling measurements is applied to flux quantification of a lysine-producing mutant of Corynebacterium glutamicum .
	manualset3
136303	6	407004	5	NULL	NULL	0	NULL	CO ( 2 ) labeling measurements	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel method for metabolic flux studies of central metabolism which is based on respirometric ( 13 ) C flux analysis , i.e. , parallel ( 13 ) C tracer studies with online CO ( 2 ) labeling measurements is applied to flux quantification of a lysine-producing mutant of Corynebacterium glutamicum .
	manualset3
136304	7	407004	5	NULL	NULL	0	NULL	flux quantification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel method for metabolic flux studies of central metabolism which is based on respirometric ( 13 ) C flux analysis , i.e. , parallel ( 13 ) C tracer studies with online CO ( 2 ) labeling measurements is applied to flux quantification of a lysine-producing mutant of Corynebacterium glutamicum .
	manualset3
136305	8	407004	5	NULL	NULL	0	NULL	lysine-producing mutant of Corynebacterium glutamicum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel method for metabolic flux studies of central metabolism which is based on respirometric ( 13 ) C flux analysis , i.e. , parallel ( 13 ) C tracer studies with online CO ( 2 ) labeling measurements is applied to flux quantification of a lysine-producing mutant of Corynebacterium glutamicum .
	manualset3
136306	1	407005	5	NULL	NULL	0	NULL	CSF concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous CSF concentrations were considerably lower , ranging from 0.04 to 0.34 mug/ml .
	manualset3
136307	2	407005	5	NULL	NULL	0	NULL	0.04 to 0.34 mug/ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous CSF concentrations were considerably lower , ranging from 0.04 to 0.34 mug/ml .
	manualset3
136308	1	407006	5	NULL	NULL	0	NULL	blood pressure measurements	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous blood pressure measurements were obtained from the arterial catheter , the oscillometric device , and the pulse oximeter .
	manualset3
136309	2	407006	5	NULL	NULL	0	NULL	arterial catheter 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous blood pressure measurements were obtained from the arterial catheter , the oscillometric device , and the pulse oximeter .
	manualset3
136310	3	407006	5	NULL	NULL	0	NULL	oscillometric device	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous blood pressure measurements were obtained from the arterial catheter , the oscillometric device , and the pulse oximeter .
	manualset3
136311	4	407006	5	NULL	NULL	0	NULL	pulse oximeter	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous blood pressure measurements were obtained from the arterial catheter , the oscillometric device , and the pulse oximeter .
	manualset3
136312	1	407007	5	NULL	NULL	0	NULL	delivery 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous delivery of the adenosine uptake inhibitors dipyridamole and S - ( 4-nitrobenzyl ) -6 - thioinosine significantly reduced evoked cortical acetylcholine release , and this effect was blocked by the simultaneous administration of caffeine .
	manualset3
136313	2	407007	5	NULL	NULL	NULL	NULL	adenosine uptake inhibitor dipyridamole	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Simultaneous delivery of the adenosine uptake inhibitors dipyridamole and S - ( 4-nitrobenzyl ) -6 - thioinosine significantly reduced evoked cortical acetylcholine release , and this effect was blocked by the simultaneous administration of caffeine .
	manualset3
136314	3	407007	5	NULL	NULL	0	NULL	adenosine uptake inhibitor S - ( 4-nitrobenzyl ) -6 - thioinosine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous delivery of the adenosine uptake inhibitors dipyridamole and S - ( 4-nitrobenzyl ) -6 - thioinosine significantly reduced evoked cortical acetylcholine release , and this effect was blocked by the simultaneous administration of caffeine .
	manualset3
136315	4	407007	5	NULL	NULL	0	NULL	cortical acetylcholine release 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous delivery of the adenosine uptake inhibitors dipyridamole and S - ( 4-nitrobenzyl ) -6 - thioinosine significantly reduced evoked cortical acetylcholine release , and this effect was blocked by the simultaneous administration of caffeine .
	manualset3
136316	5	407007	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous delivery of the adenosine uptake inhibitors dipyridamole and S - ( 4-nitrobenzyl ) -6 - thioinosine significantly reduced evoked cortical acetylcholine release , and this effect was blocked by the simultaneous administration of caffeine .
	manualset3
136317	6	407007	5	NULL	NULL	0	NULL	simultaneous administration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous delivery of the adenosine uptake inhibitors dipyridamole and S - ( 4-nitrobenzyl ) -6 - thioinosine significantly reduced evoked cortical acetylcholine release , and this effect was blocked by the simultaneous administration of caffeine .
	manualset3
136318	7	407007	5	NULL	NULL	0	NULL	caffeine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous delivery of the adenosine uptake inhibitors dipyridamole and S - ( 4-nitrobenzyl ) -6 - thioinosine significantly reduced evoked cortical acetylcholine release , and this effect was blocked by the simultaneous administration of caffeine .
	manualset3
136319	1	407008	5	NULL	NULL	0	NULL	detection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous detection of ultratrace lead and copper with gold nanoparticles patterned on carbon nanotube thin film .
	manualset3
136320	2	407008	5	NULL	NULL	0	NULL	ultratrace lead	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous detection of ultratrace lead and copper with gold nanoparticles patterned on carbon nanotube thin film .
	manualset3
136321	3	407008	5	NULL	NULL	0	NULL	copper 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous detection of ultratrace lead and copper with gold nanoparticles patterned on carbon nanotube thin film .
	manualset3
136322	4	407008	5	NULL	NULL	0	NULL	gold nanoparticles	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous detection of ultratrace lead and copper with gold nanoparticles patterned on carbon nanotube thin film .
	manualset3
136323	5	407008	5	NULL	NULL	0	NULL	carbon nanotube thin film 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous detection of ultratrace lead and copper with gold nanoparticles patterned on carbon nanotube thin film .
	manualset3
136324	1	407009	5	NULL	NULL	0	NULL	determination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous determination of disopyramide and mono-N-dealkyldisopyramide enantiomers in human plasma by capillary electrophoresis .
	manualset3
136325	2	407009	5	NULL	NULL	0	NULL	disopyramide enantiomers 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous determination of disopyramide and mono-N-dealkyldisopyramide enantiomers in human plasma by capillary electrophoresis .
	manualset3
136326	3	407009	5	NULL	NULL	0	NULL	mono-N-dealkyldisopyramide enantiomers 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous determination of disopyramide and mono-N-dealkyldisopyramide enantiomers in human plasma by capillary electrophoresis .
	manualset3
136327	4	407009	5	NULL	NULL	0	NULL	human plasma	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous determination of disopyramide and mono-N-dealkyldisopyramide enantiomers in human plasma by capillary electrophoresis .
	manualset3
136328	5	407009	5	NULL	NULL	0	NULL	capillary electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous determination of disopyramide and mono-N-dealkyldisopyramide enantiomers in human plasma by capillary electrophoresis .
	manualset3
136329	1	407010	5	NULL	NULL	0	NULL	determination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous determination of purine bases , ribonucleosides and ribonucleotides by capillary electrophoresis-electrochemistry with a copper electrode .
	manualset3
136330	2	407010	5	NULL	NULL	0	NULL	purine bases	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous determination of purine bases , ribonucleosides and ribonucleotides by capillary electrophoresis-electrochemistry with a copper electrode .
	manualset3
136331	3	407010	5	NULL	NULL	0	NULL	ribonucleosides 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous determination of purine bases , ribonucleosides and ribonucleotides by capillary electrophoresis-electrochemistry with a copper electrode .
	manualset3
136332	4	407010	5	NULL	NULL	0	NULL	ribonucleotides 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous determination of purine bases , ribonucleosides and ribonucleotides by capillary electrophoresis-electrochemistry with a copper electrode .
	manualset3
136333	5	407010	5	NULL	NULL	0	NULL	capillary electrophoresis-electrochemistry 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous determination of purine bases , ribonucleosides and ribonucleotides by capillary electrophoresis-electrochemistry with a copper electrode .
	manualset3
136334	6	407010	5	NULL	NULL	0	NULL	copper electrode	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous determination of purine bases , ribonucleosides and ribonucleotides by capillary electrophoresis-electrochemistry with a copper electrode .
	manualset3
136335	1	407011	5	NULL	NULL	0	NULL	flow cytometry measurements	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous flow cytometry measurements revealed that ERK , p38 MAPK and JNK were phosphorylated as early as 5 min after IL-6 injection .
	manualset3
136336	2	407011	5	NULL	NULL	0	NULL	ERK 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous flow cytometry measurements revealed that ERK , p38 MAPK and JNK were phosphorylated as early as 5 min after IL-6 injection .
	manualset3
136337	3	407011	5	NULL	NULL	0	NULL	p38 MAPK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous flow cytometry measurements revealed that ERK , p38 MAPK and JNK were phosphorylated as early as 5 min after IL-6 injection .
	manualset3
136338	4	407011	5	NULL	NULL	0	NULL	JNK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous flow cytometry measurements revealed that ERK , p38 MAPK and JNK were phosphorylated as early as 5 min after IL-6 injection .
	manualset3
136339	5	407011	5	NULL	NULL	0	NULL	5 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous flow cytometry measurements revealed that ERK , p38 MAPK and JNK were phosphorylated as early as 5 min after IL-6 injection .
	manualset3
136340	6	407011	5	NULL	NULL	0	NULL	 IL-6 injection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous flow cytometry measurements revealed that ERK , p38 MAPK and JNK were phosphorylated as early as 5 min after IL-6 injection .
	manualset3
136341	1	407012	5	NULL	NULL	0	NULL	presentation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous presentation of renal cell carcinoma and primary breast carcinoma -- a rare occurrence ?
	manualset3
136342	2	407012	5	NULL	NULL	0	NULL	renal cell carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous presentation of renal cell carcinoma and primary breast carcinoma -- a rare occurrence ?
	manualset3
136343	3	407012	5	NULL	NULL	0	NULL	primary breast carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous presentation of renal cell carcinoma and primary breast carcinoma -- a rare occurrence ?
	manualset3
136344	4	407012	5	NULL	NULL	0	NULL	occurrence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous presentation of renal cell carcinoma and primary breast carcinoma -- a rare occurrence ?
	manualset3
136345	1	407013	5	NULL	NULL	0	NULL	treatment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous treatment with both OA-Alb and acidic media led to phosphorylation of the intracellular pH sensor Pyk2 .
	manualset3
136347	2	407013	5	NULL	NULL	0	NULL	OA-Alb media	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous treatment with both OA-Alb and acidic media led to phosphorylation of the intracellular pH sensor Pyk2 .
	manualset3
136349	3	407013	5	NULL	NULL	0	NULL	acidic media 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous treatment with both OA-Alb and acidic media led to phosphorylation of the intracellular pH sensor Pyk2 .
	manualset3
136351	4	407013	5	NULL	NULL	0	NULL	phosphorylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous treatment with both OA-Alb and acidic media led to phosphorylation of the intracellular pH sensor Pyk2 .
	manualset3
136354	5	407013	5	NULL	NULL	0	NULL	intracellular pH sensor Pyk2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous treatment with both OA-Alb and acidic media led to phosphorylation of the intracellular pH sensor Pyk2 .
	manualset3
136356	1	407014	5	NULL	NULL	0	NULL	LPO 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneously , LPO increased by 78 % , PCG by 60 % , AOPP by 84 % , and NO ( 2 ) by 70 % .
	manualset3
136357	2	407014	5	NULL	NULL	0	NULL	78 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneously , LPO increased by 78 % , PCG by 60 % , AOPP by 84 % , and NO ( 2 ) by 70 % .
	manualset3
136358	3	407014	5	NULL	NULL	0	NULL	PCG	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneously , LPO increased by 78 % , PCG by 60 % , AOPP by 84 % , and NO ( 2 ) by 70 % .
	manualset3
136359	4	407014	5	NULL	NULL	0	NULL	60 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneously , LPO increased by 78 % , PCG by 60 % , AOPP by 84 % , and NO ( 2 ) by 70 % .
	manualset3
136360	5	407014	5	NULL	NULL	0	NULL	AOPP 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneously , LPO increased by 78 % , PCG by 60 % , AOPP by 84 % , and NO ( 2 ) by 70 % .
	manualset3
136361	6	407014	5	NULL	NULL	0	NULL	84 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneously , LPO increased by 78 % , PCG by 60 % , AOPP by 84 % , and NO ( 2 ) by 70 % .
	manualset3
136362	7	407014	5	NULL	NULL	0	NULL	NO ( 2 ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneously , LPO increased by 78 % , PCG by 60 % , AOPP by 84 % , and NO ( 2 ) by 70 % .
	manualset3
136363	8	407014	5	NULL	NULL	0	NULL	70 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneously , LPO increased by 78 % , PCG by 60 % , AOPP by 84 % , and NO ( 2 ) by 70 % .
	manualset3
136364	1	407015	5	NULL	NULL	0	NULL	cardiac output 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneously , cardiac output increased , but left ventricular end-diastolic pressure , dP/dt , and dP/dt/P did not change significantly .
	manualset3
136365	2	407015	5	NULL	NULL	0	NULL	left ventricular end-diastolic pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneously , cardiac output increased , but left ventricular end-diastolic pressure , dP/dt , and dP/dt/P did not change significantly .
	manualset3
136366	3	407015	5	NULL	NULL	0	NULL	dP/dt	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneously , cardiac output increased , but left ventricular end-diastolic pressure , dP/dt , and dP/dt/P did not change significantly .
	manualset3
136367	4	407015	5	NULL	NULL	0	NULL	dP/dt/P	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneously , cardiac output increased , but left ventricular end-diastolic pressure , dP/dt , and dP/dt/P did not change significantly .
	manualset3
136368	1	407016	5	NULL	NULL	0	NULL	Simvastatin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Simvastatin at the dosage of 10 mg appeared to be at least as efficient as 12 g of cholestyramine and generally better tolerated .
	manualset3
136369	2	407016	5	NULL	NULL	0	NULL	dosage 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Simvastatin at the dosage of 10 mg appeared to be at least as efficient as 12 g of cholestyramine and generally better tolerated .
	manualset3
136370	3	407016	5	NULL	NULL	0	NULL	10 mg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Simvastatin at the dosage of 10 mg appeared to be at least as efficient as 12 g of cholestyramine and generally better tolerated .
	manualset3
136371	4	407016	5	NULL	NULL	0	NULL	12 g	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Simvastatin at the dosage of 10 mg appeared to be at least as efficient as 12 g of cholestyramine and generally better tolerated .
	manualset3
136372	5	407016	5	NULL	NULL	0	NULL	cholestyramine 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Simvastatin at the dosage of 10 mg appeared to be at least as efficient as 12 g of cholestyramine and generally better tolerated .
	manualset3
136373	1	407017	5	NULL	NULL	0	NULL	Simvastatin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Simvastatin intensifies heart rate depression after metoprolol and atropine administration in normocholesterolemic rats .
	manualset3
136374	2	407017	5	NULL	NULL	0	NULL	heart rate depression	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Simvastatin intensifies heart rate depression after metoprolol and atropine administration in normocholesterolemic rats .
	manualset3
136375	3	407017	5	NULL	NULL	0	NULL	metoprolol administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Simvastatin intensifies heart rate depression after metoprolol and atropine administration in normocholesterolemic rats .
	manualset3
136376	4	407017	5	NULL	NULL	0	NULL	atropine administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Simvastatin intensifies heart rate depression after metoprolol and atropine administration in normocholesterolemic rats .
	manualset3
136378	5	407017	5	NULL	NULL	0	NULL	normocholesterolemic rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Simvastatin intensifies heart rate depression after metoprolol and atropine administration in normocholesterolemic rats .
	manualset3
136404	1	407018	5	NULL	NULL	0	NULL	1991 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Since 1991 , most of the determined substances ( e.g. sulfate , nitrate , calcium , lead , benzo ( a ) pyrene , alpha-HCH ) show decreased concentration values in bark samples from both sites .
	manualset3
136406	2	407018	5	NULL	NULL	0	NULL	determined substances	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Since 1991 , most of the determined substances ( e.g. sulfate , nitrate , calcium , lead , benzo ( a ) pyrene , alpha-HCH ) show decreased concentration values in bark samples from both sites .
	manualset3
136407	3	407018	5	NULL	NULL	0	NULL	sulfate 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Since 1991 , most of the determined substances ( e.g. sulfate , nitrate , calcium , lead , benzo ( a ) pyrene , alpha-HCH ) show decreased concentration values in bark samples from both sites .
	manualset3
136408	4	407018	5	NULL	NULL	0	NULL	nitrate 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Since 1991 , most of the determined substances ( e.g. sulfate , nitrate , calcium , lead , benzo ( a ) pyrene , alpha-HCH ) show decreased concentration values in bark samples from both sites .
	manualset3
136409	5	407018	5	NULL	NULL	0	NULL	calcium 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Since 1991 , most of the determined substances ( e.g. sulfate , nitrate , calcium , lead , benzo ( a ) pyrene , alpha-HCH ) show decreased concentration values in bark samples from both sites .
	manualset3
136410	6	407018	5	NULL	NULL	0	NULL	lead 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Since 1991 , most of the determined substances ( e.g. sulfate , nitrate , calcium , lead , benzo ( a ) pyrene , alpha-HCH ) show decreased concentration values in bark samples from both sites .
	manualset3
136411	7	407018	5	NULL	NULL	0	NULL	benzo ( a ) pyrene	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Since 1991 , most of the determined substances ( e.g. sulfate , nitrate , calcium , lead , benzo ( a ) pyrene , alpha-HCH ) show decreased concentration values in bark samples from both sites .
	manualset3
136412	8	407018	5	NULL	NULL	0	NULL	alpha-HCH	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Since 1991 , most of the determined substances ( e.g. sulfate , nitrate , calcium , lead , benzo ( a ) pyrene , alpha-HCH ) show decreased concentration values in bark samples from both sites .
	manualset3
136413	9	407018	5	NULL	NULL	0	NULL	concentration values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since 1991 , most of the determined substances ( e.g. sulfate , nitrate , calcium , lead , benzo ( a ) pyrene , alpha-HCH ) show decreased concentration values in bark samples from both sites .
	manualset3
136419	10	407018	5	NULL	NULL	0	NULL	bark samples	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Since 1991 , most of the determined substances ( e.g. sulfate , nitrate , calcium , lead , benzo ( a ) pyrene , alpha-HCH ) show decreased concentration values in bark samples from both sites .
	manualset3
136420	11	407018	5	NULL	NULL	0	NULL	sites 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since 1991 , most of the determined substances ( e.g. sulfate , nitrate , calcium , lead , benzo ( a ) pyrene , alpha-HCH ) show decreased concentration values in bark samples from both sites .
	manualset3
136421	1	407019	5	NULL	NULL	0	NULL	70 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Since 70 % of hospital costs are personnel costs , a substantial reduction in the hospital budget can only be obtained by reducing staff .
	manualset3
136422	2	407019	5	NULL	NULL	0	NULL	hospital costs	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since 70 % of hospital costs are personnel costs , a substantial reduction in the hospital budget can only be obtained by reducing staff .
	manualset3
136423	3	407019	5	NULL	NULL	0	NULL	personnel costs	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since 70 % of hospital costs are personnel costs , a substantial reduction in the hospital budget can only be obtained by reducing staff .
	manualset3
136424	4	407019	5	NULL	NULL	0	NULL	substantial reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since 70 % of hospital costs are personnel costs , a substantial reduction in the hospital budget can only be obtained by reducing staff .
	manualset3
136425	5	407019	5	NULL	NULL	0	NULL	hospital budget	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since 70 % of hospital costs are personnel costs , a substantial reduction in the hospital budget can only be obtained by reducing staff .
	manualset3
136426	6	407019	5	NULL	NULL	0	NULL	staff 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since 70 % of hospital costs are personnel costs , a substantial reduction in the hospital budget can only be obtained by reducing staff .
	manualset3
136427	1	407020	5	NULL	NULL	0	NULL	novel synthesis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel synthesis of optically-active alpha-alanine .
	manualset3
136428	2	407020	5	NULL	NULL	0	NULL	optically-active alpha-alanine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel synthesis of optically-active alpha-alanine .
	manualset3
136430	1	407021	5	NULL	NULL	NULL	NULL	C3X	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Since C3X was obtained by elution with a high salt solution from TAK incubated with ethylenediaminetetraacetate ( EDTA ) - serum ( serum containing EDTA ) but not from TAK incubated with EDTA-plasma , C3X could already be present in the serum before the activation of ACP by TAK .
	manualset3
136432	2	407021	5	NULL	NULL	0	NULL	elution 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since C3X was obtained by elution with a high salt solution from TAK incubated with ethylenediaminetetraacetate ( EDTA ) - serum ( serum containing EDTA ) but not from TAK incubated with EDTA-plasma , C3X could already be present in the serum before the activation of ACP by TAK .
	manualset3
136433	3	407021	5	NULL	NULL	0	NULL	high salt solution 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Since C3X was obtained by elution with a high salt solution from TAK incubated with ethylenediaminetetraacetate ( EDTA ) - serum ( serum containing EDTA ) but not from TAK incubated with EDTA-plasma , C3X could already be present in the serum before the activation of ACP by TAK .
	manualset3
136435	4	407021	5	NULL	NULL	0	NULL	TAK 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since C3X was obtained by elution with a high salt solution from TAK incubated with ethylenediaminetetraacetate ( EDTA ) - serum ( serum containing EDTA ) but not from TAK incubated with EDTA-plasma , C3X could already be present in the serum before the activation of ACP by TAK .
	manualset3
136439	5	407021	5	NULL	NULL	0	NULL	ethylenediaminetetraacetate ( EDTA ) - serum ( serum containing EDTA ) 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Since C3X was obtained by elution with a high salt solution from TAK incubated with ethylenediaminetetraacetate ( EDTA ) - serum ( serum containing EDTA ) but not from TAK incubated with EDTA-plasma , C3X could already be present in the serum before the activation of ACP by TAK .
	manualset3
136440	6	407021	5	NULL	NULL	0	NULL	TAK 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Since C3X was obtained by elution with a high salt solution from TAK incubated with ethylenediaminetetraacetate ( EDTA ) - serum ( serum containing EDTA ) but not from TAK incubated with EDTA-plasma , C3X could already be present in the serum before the activation of ACP by TAK .
	manualset3
136441	7	407021	5	NULL	NULL	0	NULL	EDTA-plasma	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Since C3X was obtained by elution with a high salt solution from TAK incubated with ethylenediaminetetraacetate ( EDTA ) - serum ( serum containing EDTA ) but not from TAK incubated with EDTA-plasma , C3X could already be present in the serum before the activation of ACP by TAK .
	manualset3
136442	8	407021	5	NULL	NULL	0	NULL	C3X 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Since C3X was obtained by elution with a high salt solution from TAK incubated with ethylenediaminetetraacetate ( EDTA ) - serum ( serum containing EDTA ) but not from TAK incubated with EDTA-plasma , C3X could already be present in the serum before the activation of ACP by TAK .
	manualset3
136443	9	407021	5	NULL	NULL	0	NULL	serum 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Since C3X was obtained by elution with a high salt solution from TAK incubated with ethylenediaminetetraacetate ( EDTA ) - serum ( serum containing EDTA ) but not from TAK incubated with EDTA-plasma , C3X could already be present in the serum before the activation of ACP by TAK .
	manualset3
136444	10	407021	5	NULL	NULL	0	NULL	activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since C3X was obtained by elution with a high salt solution from TAK incubated with ethylenediaminetetraacetate ( EDTA ) - serum ( serum containing EDTA ) but not from TAK incubated with EDTA-plasma , C3X could already be present in the serum before the activation of ACP by TAK .
	manualset3
136445	11	407021	5	NULL	NULL	0	NULL	ACP 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since C3X was obtained by elution with a high salt solution from TAK incubated with ethylenediaminetetraacetate ( EDTA ) - serum ( serum containing EDTA ) but not from TAK incubated with EDTA-plasma , C3X could already be present in the serum before the activation of ACP by TAK .
	manualset3
136446	12	407021	5	NULL	NULL	0	NULL	TAK 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Since C3X was obtained by elution with a high salt solution from TAK incubated with ethylenediaminetetraacetate ( EDTA ) - serum ( serum containing EDTA ) but not from TAK incubated with EDTA-plasma , C3X could already be present in the serum before the activation of ACP by TAK .
	manualset3
136447	1	407022	5	NULL	NULL	0	NULL	IL-6 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Since IL-6 is a potent stimulator of megakaryocytopoiesis we examined IL-6 production at the tumor site and its relationship to serum IL-6 levels and circulating platelet counts in patients with ovarian cancer .
	manualset3
136448	2	407022	5	NULL	NULL	0	NULL	potent stimulator	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Since IL-6 is a potent stimulator of megakaryocytopoiesis we examined IL-6 production at the tumor site and its relationship to serum IL-6 levels and circulating platelet counts in patients with ovarian cancer .
	manualset3
136449	3	407022	5	NULL	NULL	0	NULL	megakaryocytopoiesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since IL-6 is a potent stimulator of megakaryocytopoiesis we examined IL-6 production at the tumor site and its relationship to serum IL-6 levels and circulating platelet counts in patients with ovarian cancer .
	manualset3
136450	4	407022	5	NULL	NULL	0	NULL	IL-6 production 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since IL-6 is a potent stimulator of megakaryocytopoiesis we examined IL-6 production at the tumor site and its relationship to serum IL-6 levels and circulating platelet counts in patients with ovarian cancer .
	manualset3
136451	5	407022	5	NULL	NULL	0	NULL	tumor site	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Since IL-6 is a potent stimulator of megakaryocytopoiesis we examined IL-6 production at the tumor site and its relationship to serum IL-6 levels and circulating platelet counts in patients with ovarian cancer .
	manualset3
136453	6	407022	5	NULL	NULL	0	NULL	relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Since IL-6 is a potent stimulator of megakaryocytopoiesis we examined IL-6 production at the tumor site and its relationship to serum IL-6 levels and circulating platelet counts in patients with ovarian cancer .
	manualset3
136455	7	407022	5	NULL	NULL	0	NULL	serum IL-6 levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since IL-6 is a potent stimulator of megakaryocytopoiesis we examined IL-6 production at the tumor site and its relationship to serum IL-6 levels and circulating platelet counts in patients with ovarian cancer .
	manualset3
136456	8	407022	5	NULL	NULL	0	NULL	circulating platelet counts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since IL-6 is a potent stimulator of megakaryocytopoiesis we examined IL-6 production at the tumor site and its relationship to serum IL-6 levels and circulating platelet counts in patients with ovarian cancer .
	manualset3
136458	9	407022	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since IL-6 is a potent stimulator of megakaryocytopoiesis we examined IL-6 production at the tumor site and its relationship to serum IL-6 levels and circulating platelet counts in patients with ovarian cancer .
	manualset3
136459	10	407022	5	NULL	NULL	0	NULL	ovarian cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Since IL-6 is a potent stimulator of megakaryocytopoiesis we examined IL-6 production at the tumor site and its relationship to serum IL-6 levels and circulating platelet counts in patients with ovarian cancer .
	manualset3
136460	1	407023	5	NULL	NULL	0	NULL	June 2007	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Since June 2007 , this patient has complained of hematuria and bloody stool .
	manualset3
136461	2	407023	5	NULL	NULL	0	NULL	patient 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since June 2007 , this patient has complained of hematuria and bloody stool .
	manualset3
136462	3	407023	5	NULL	NULL	0	NULL	hematuria 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since June 2007 , this patient has complained of hematuria and bloody stool .
	manualset3
136463	4	407023	5	NULL	NULL	0	NULL	bloody stool 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since June 2007 , this patient has complained of hematuria and bloody stool .
	manualset3
136467	1	407024	5	NULL	NULL	0	NULL	M stars	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since M stars are active at the X-ray and extreme ultraviolet radiation ( XUV ) wave-lengths over long periods of time , we have applied a thermal balance model at various XUV flux input values for simulating the thermospheric heating by photodissociation and ionization processes due to exothermic chemical reactions and cooling by the CO2 infrared radiation in the 15 microm band .
	manualset3
136468	2	407024	5	NULL	NULL	NULL	NULL	X-ray wave-lengths	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Since M stars are active at the X-ray and extreme ultraviolet radiation ( XUV ) wave-lengths over long periods of time , we have applied a thermal balance model at various XUV flux input values for simulating the thermospheric heating by photodissociation and ionization processes due to exothermic chemical reactions and cooling by the CO2 infrared radiation in the 15 microm band .
	manualset3
136469	3	407024	5	NULL	NULL	0	NULL	extreme ultraviolet radiation ( XUV ) wave-lengths	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since M stars are active at the X-ray and extreme ultraviolet radiation ( XUV ) wave-lengths over long periods of time , we have applied a thermal balance model at various XUV flux input values for simulating the thermospheric heating by photodissociation and ionization processes due to exothermic chemical reactions and cooling by the CO2 infrared radiation in the 15 microm band .
	manualset3
136470	4	407024	5	NULL	NULL	0	NULL	long periods	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Since M stars are active at the X-ray and extreme ultraviolet radiation ( XUV ) wave-lengths over long periods of time , we have applied a thermal balance model at various XUV flux input values for simulating the thermospheric heating by photodissociation and ionization processes due to exothermic chemical reactions and cooling by the CO2 infrared radiation in the 15 microm band .
	manualset3
136471	5	407024	5	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Since M stars are active at the X-ray and extreme ultraviolet radiation ( XUV ) wave-lengths over long periods of time , we have applied a thermal balance model at various XUV flux input values for simulating the thermospheric heating by photodissociation and ionization processes due to exothermic chemical reactions and cooling by the CO2 infrared radiation in the 15 microm band .
	manualset3
136472	6	407024	5	NULL	NULL	0	NULL	thermal balance model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Since M stars are active at the X-ray and extreme ultraviolet radiation ( XUV ) wave-lengths over long periods of time , we have applied a thermal balance model at various XUV flux input values for simulating the thermospheric heating by photodissociation and ionization processes due to exothermic chemical reactions and cooling by the CO2 infrared radiation in the 15 microm band .
	manualset3
136473	7	407024	5	NULL	NULL	0	NULL	XUV flux input values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since M stars are active at the X-ray and extreme ultraviolet radiation ( XUV ) wave-lengths over long periods of time , we have applied a thermal balance model at various XUV flux input values for simulating the thermospheric heating by photodissociation and ionization processes due to exothermic chemical reactions and cooling by the CO2 infrared radiation in the 15 microm band .
	manualset3
136474	8	407024	5	NULL	NULL	0	NULL	thermospheric heating	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since M stars are active at the X-ray and extreme ultraviolet radiation ( XUV ) wave-lengths over long periods of time , we have applied a thermal balance model at various XUV flux input values for simulating the thermospheric heating by photodissociation and ionization processes due to exothermic chemical reactions and cooling by the CO2 infrared radiation in the 15 microm band .
	manualset3
136475	9	407024	5	NULL	NULL	NULL	NULL	photodissociation 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Since M stars are active at the X-ray and extreme ultraviolet radiation ( XUV ) wave-lengths over long periods of time , we have applied a thermal balance model at various XUV flux input values for simulating the thermospheric heating by photodissociation and ionization processes due to exothermic chemical reactions and cooling by the CO2 infrared radiation in the 15 microm band .
	manualset3
136476	10	407024	5	NULL	NULL	NULL	NULL	ionization processes	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Since M stars are active at the X-ray and extreme ultraviolet radiation ( XUV ) wave-lengths over long periods of time , we have applied a thermal balance model at various XUV flux input values for simulating the thermospheric heating by photodissociation and ionization processes due to exothermic chemical reactions and cooling by the CO2 infrared radiation in the 15 microm band .
	manualset3
136477	11	407024	5	NULL	NULL	0	NULL	exothermic chemical reactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since M stars are active at the X-ray and extreme ultraviolet radiation ( XUV ) wave-lengths over long periods of time , we have applied a thermal balance model at various XUV flux input values for simulating the thermospheric heating by photodissociation and ionization processes due to exothermic chemical reactions and cooling by the CO2 infrared radiation in the 15 microm band .
	manualset3
136478	12	407024	5	NULL	NULL	0	NULL	cooling 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since M stars are active at the X-ray and extreme ultraviolet radiation ( XUV ) wave-lengths over long periods of time , we have applied a thermal balance model at various XUV flux input values for simulating the thermospheric heating by photodissociation and ionization processes due to exothermic chemical reactions and cooling by the CO2 infrared radiation in the 15 microm band .
	manualset3
136479	13	407024	5	NULL	NULL	0	NULL	CO2 infrared radiation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Since M stars are active at the X-ray and extreme ultraviolet radiation ( XUV ) wave-lengths over long periods of time , we have applied a thermal balance model at various XUV flux input values for simulating the thermospheric heating by photodissociation and ionization processes due to exothermic chemical reactions and cooling by the CO2 infrared radiation in the 15 microm band .
	manualset3
136480	14	407024	5	NULL	NULL	0	NULL	15 microm band	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since M stars are active at the X-ray and extreme ultraviolet radiation ( XUV ) wave-lengths over long periods of time , we have applied a thermal balance model at various XUV flux input values for simulating the thermospheric heating by photodissociation and ionization processes due to exothermic chemical reactions and cooling by the CO2 infrared radiation in the 15 microm band .
	manualset3
136481	1	407025	5	NULL	NULL	0	NULL	 NF-B activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since NF-B activation is implicated in asthma pathogenesis , we investigated whether AKR1B1 inhibition could prevent ovalbumin ( Ova ) - and ragweed pollen extract ( RWE ) - induced airway inflammation and hyper-responsiveness in mice models and tumor necrosis factor-alpha ( TNF - ) - , lipopolysachharide ( LPS ) - and RWE-induced cytotoxic and inflammatory signals in primary human small airway epithelial cells ( SAEC ) .
	manualset3
136482	2	407025	5	NULL	NULL	0	NULL	asthma pathogenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since NF-B activation is implicated in asthma pathogenesis , we investigated whether AKR1B1 inhibition could prevent ovalbumin ( Ova ) - and ragweed pollen extract ( RWE ) - induced airway inflammation and hyper-responsiveness in mice models and tumor necrosis factor-alpha ( TNF - ) - , lipopolysachharide ( LPS ) - and RWE-induced cytotoxic and inflammatory signals in primary human small airway epithelial cells ( SAEC ) .
	manualset3
136483	3	407025	5	NULL	NULL	0	NULL	AKR1B1 inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since NF-B activation is implicated in asthma pathogenesis , we investigated whether AKR1B1 inhibition could prevent ovalbumin ( Ova ) - and ragweed pollen extract ( RWE ) - induced airway inflammation and hyper-responsiveness in mice models and tumor necrosis factor-alpha ( TNF - ) - , lipopolysachharide ( LPS ) - and RWE-induced cytotoxic and inflammatory signals in primary human small airway epithelial cells ( SAEC ) .
	manualset3
136484	4	407025	5	NULL	NULL	0	NULL	ovalbumin ( Ova ) - induced airway inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since NF-B activation is implicated in asthma pathogenesis , we investigated whether AKR1B1 inhibition could prevent ovalbumin ( Ova ) - and ragweed pollen extract ( RWE ) - induced airway inflammation and hyper-responsiveness in mice models and tumor necrosis factor-alpha ( TNF - ) - , lipopolysachharide ( LPS ) - and RWE-induced cytotoxic and inflammatory signals in primary human small airway epithelial cells ( SAEC ) .
	manualset3
136486	5	407025	5	NULL	NULL	0	NULL	ragweed pollen extract ( RWE ) - induced airway inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since NF-B activation is implicated in asthma pathogenesis , we investigated whether AKR1B1 inhibition could prevent ovalbumin ( Ova ) - and ragweed pollen extract ( RWE ) - induced airway inflammation and hyper-responsiveness in mice models and tumor necrosis factor-alpha ( TNF - ) - , lipopolysachharide ( LPS ) - and RWE-induced cytotoxic and inflammatory signals in primary human small airway epithelial cells ( SAEC ) .
	manualset3
136487	6	407025	5	NULL	NULL	0	NULL	hyper-responsiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since NF-B activation is implicated in asthma pathogenesis , we investigated whether AKR1B1 inhibition could prevent ovalbumin ( Ova ) - and ragweed pollen extract ( RWE ) - induced airway inflammation and hyper-responsiveness in mice models and tumor necrosis factor-alpha ( TNF - ) - , lipopolysachharide ( LPS ) - and RWE-induced cytotoxic and inflammatory signals in primary human small airway epithelial cells ( SAEC ) .
	manualset3
136490	7	407025	5	NULL	NULL	0	NULL	mice models	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Since NF-B activation is implicated in asthma pathogenesis , we investigated whether AKR1B1 inhibition could prevent ovalbumin ( Ova ) - and ragweed pollen extract ( RWE ) - induced airway inflammation and hyper-responsiveness in mice models and tumor necrosis factor-alpha ( TNF - ) - , lipopolysachharide ( LPS ) - and RWE-induced cytotoxic and inflammatory signals in primary human small airway epithelial cells ( SAEC ) .
	manualset3
136492	8	407025	5	NULL	NULL	0	NULL	tumor necrosis factor-alpha ( TNF - ) -induced cytotoxic and inflammatory signals 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since NF-B activation is implicated in asthma pathogenesis , we investigated whether AKR1B1 inhibition could prevent ovalbumin ( Ova ) - and ragweed pollen extract ( RWE ) - induced airway inflammation and hyper-responsiveness in mice models and tumor necrosis factor-alpha ( TNF - ) - , lipopolysachharide ( LPS ) - and RWE-induced cytotoxic and inflammatory signals in primary human small airway epithelial cells ( SAEC ) .
	manualset3
136494	9	407025	5	NULL	NULL	0	NULL	lipopolysachharide ( LPS ) -induced cytotoxic and inflammatory signals	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since NF-B activation is implicated in asthma pathogenesis , we investigated whether AKR1B1 inhibition could prevent ovalbumin ( Ova ) - and ragweed pollen extract ( RWE ) - induced airway inflammation and hyper-responsiveness in mice models and tumor necrosis factor-alpha ( TNF - ) - , lipopolysachharide ( LPS ) - and RWE-induced cytotoxic and inflammatory signals in primary human small airway epithelial cells ( SAEC ) .
	manualset3
136497	10	407025	5	NULL	NULL	0	NULL	RWE-induced cytotoxic and inflammatory signals	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since NF-B activation is implicated in asthma pathogenesis , we investigated whether AKR1B1 inhibition could prevent ovalbumin ( Ova ) - and ragweed pollen extract ( RWE ) - induced airway inflammation and hyper-responsiveness in mice models and tumor necrosis factor-alpha ( TNF - ) - , lipopolysachharide ( LPS ) - and RWE-induced cytotoxic and inflammatory signals in primary human small airway epithelial cells ( SAEC ) .
	manualset3
136498	11	407025	5	NULL	NULL	0	NULL	primary human small airway epithelial cells ( SAEC )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Since NF-B activation is implicated in asthma pathogenesis , we investigated whether AKR1B1 inhibition could prevent ovalbumin ( Ova ) - and ragweed pollen extract ( RWE ) - induced airway inflammation and hyper-responsiveness in mice models and tumor necrosis factor-alpha ( TNF - ) - , lipopolysachharide ( LPS ) - and RWE-induced cytotoxic and inflammatory signals in primary human small airway epithelial cells ( SAEC ) .
	manualset3
136501	1	407026	5	NULL	NULL	0	NULL	NF-kappa B induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since NF-kappa B induction occurs as a response to stress and p53 arrests cells in G1/S , where repair may be initiated , activation of p53 by NF-kappa B could be a mechanism by which cells can recover from stress .
	manualset3
136502	2	407026	5	NULL	NULL	0	NULL	response 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since NF-kappa B induction occurs as a response to stress and p53 arrests cells in G1/S , where repair may be initiated , activation of p53 by NF-kappa B could be a mechanism by which cells can recover from stress .
	manualset3
136503	3	407026	5	NULL	NULL	0	NULL	stress 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since NF-kappa B induction occurs as a response to stress and p53 arrests cells in G1/S , where repair may be initiated , activation of p53 by NF-kappa B could be a mechanism by which cells can recover from stress .
	manualset3
136504	4	407026	5	NULL	NULL	0	NULL	p53 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Since NF-kappa B induction occurs as a response to stress and p53 arrests cells in G1/S , where repair may be initiated , activation of p53 by NF-kappa B could be a mechanism by which cells can recover from stress .
	manualset3
136505	5	407026	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Since NF-kappa B induction occurs as a response to stress and p53 arrests cells in G1/S , where repair may be initiated , activation of p53 by NF-kappa B could be a mechanism by which cells can recover from stress .
	manualset3
136506	6	407026	5	NULL	NULL	0	NULL	G1/S	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Since NF-kappa B induction occurs as a response to stress and p53 arrests cells in G1/S , where repair may be initiated , activation of p53 by NF-kappa B could be a mechanism by which cells can recover from stress .
	manualset3
136507	7	407026	5	NULL	NULL	0	NULL	repair 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since NF-kappa B induction occurs as a response to stress and p53 arrests cells in G1/S , where repair may be initiated , activation of p53 by NF-kappa B could be a mechanism by which cells can recover from stress .
	manualset3
136508	8	407026	5	NULL	NULL	0	NULL	activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since NF-kappa B induction occurs as a response to stress and p53 arrests cells in G1/S , where repair may be initiated , activation of p53 by NF-kappa B could be a mechanism by which cells can recover from stress .
	manualset3
136509	9	407026	5	NULL	NULL	NULL	NULL	p53 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Since NF-kappa B induction occurs as a response to stress and p53 arrests cells in G1/S , where repair may be initiated , activation of p53 by NF-kappa B could be a mechanism by which cells can recover from stress .
	manualset3
136510	10	407026	5	NULL	NULL	0	NULL	NF-kappa B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Since NF-kappa B induction occurs as a response to stress and p53 arrests cells in G1/S , where repair may be initiated , activation of p53 by NF-kappa B could be a mechanism by which cells can recover from stress .
	manualset3
136511	11	407026	5	NULL	NULL	0	NULL	mechanism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since NF-kappa B induction occurs as a response to stress and p53 arrests cells in G1/S , where repair may be initiated , activation of p53 by NF-kappa B could be a mechanism by which cells can recover from stress .
	manualset3
136513	12	407026	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Since NF-kappa B induction occurs as a response to stress and p53 arrests cells in G1/S , where repair may be initiated , activation of p53 by NF-kappa B could be a mechanism by which cells can recover from stress .
	manualset3
136517	13	407026	5	NULL	NULL	0	NULL	stress 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since NF-kappa B induction occurs as a response to stress and p53 arrests cells in G1/S , where repair may be initiated , activation of p53 by NF-kappa B could be a mechanism by which cells can recover from stress .
	manualset3
136522	1	407027	5	NULL	NULL	0	NULL	NO 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Since NO has been shown to increase the level of cGMP in other cell types , we used 8-Br-cGMP in order to mimic the effects of NO. .
	manualset3
136525	3	407027	5	NULL	NULL	0	NULL	level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since NO has been shown to increase the level of cGMP in other cell types , we used 8-Br-cGMP in order to mimic the effects of NO. .
	manualset3
136526	4	407027	5	NULL	NULL	0	NULL	cGMP 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Since NO has been shown to increase the level of cGMP in other cell types , we used 8-Br-cGMP in order to mimic the effects of NO. .
	manualset3
136527	5	407027	5	NULL	NULL	0	NULL	cell types	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Since NO has been shown to increase the level of cGMP in other cell types , we used 8-Br-cGMP in order to mimic the effects of NO. .
	manualset3
136529	6	407027	5	NULL	NULL	0	NULL	8-Br-cGMP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Since NO has been shown to increase the level of cGMP in other cell types , we used 8-Br-cGMP in order to mimic the effects of NO. .
	manualset3
136530	7	407027	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since NO has been shown to increase the level of cGMP in other cell types , we used 8-Br-cGMP in order to mimic the effects of NO. .
	manualset3
136532	8	407027	5	NULL	NULL	0	NULL	NO	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Since NO has been shown to increase the level of cGMP in other cell types , we used 8-Br-cGMP in order to mimic the effects of NO. .
	manualset3
136535	1	407028	5	NULL	NULL	NULL	NULL	 TNF-alpha inhibitors	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Since TNF-alpha inhibitors have been used in Korea , a few cases of TNF-alpha inhibitor associated tuberculosis have been described .
	manualset3
136536	2	407028	5	NULL	NULL	0	NULL	Korea 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Since TNF-alpha inhibitors have been used in Korea , a few cases of TNF-alpha inhibitor associated tuberculosis have been described .
	manualset3
136537	3	407028	5	NULL	NULL	NULL	NULL	cases 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Since TNF-alpha inhibitors have been used in Korea , a few cases of TNF-alpha inhibitor associated tuberculosis have been described .
	manualset3
136538	4	407028	5	NULL	NULL	0	NULL	 TNF-alpha inhibitor associated tuberculosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Since TNF-alpha inhibitors have been used in Korea , a few cases of TNF-alpha inhibitor associated tuberculosis have been described .
	manualset3
136539	1	407029	5	NULL	NULL	0	NULL	basic fibroblast growth factor ( bFGF ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Since basic fibroblast growth factor ( bFGF ) enhances the survival and growth of dopaminergic neurons in vitro , we explored whether cells genetically modified to produce bFGF would improve the functional efficacy of dopaminergic neurons implanted into rats with experimental Parkinson 's disease .
	manualset3
136540	2	407029	5	NULL	NULL	0	NULL	survival 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since basic fibroblast growth factor ( bFGF ) enhances the survival and growth of dopaminergic neurons in vitro , we explored whether cells genetically modified to produce bFGF would improve the functional efficacy of dopaminergic neurons implanted into rats with experimental Parkinson 's disease .
	manualset3
136541	3	407029	5	NULL	NULL	0	NULL	growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since basic fibroblast growth factor ( bFGF ) enhances the survival and growth of dopaminergic neurons in vitro , we explored whether cells genetically modified to produce bFGF would improve the functional efficacy of dopaminergic neurons implanted into rats with experimental Parkinson 's disease .
	manualset3
136542	4	407029	5	NULL	NULL	0	NULL	dopaminergic neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Since basic fibroblast growth factor ( bFGF ) enhances the survival and growth of dopaminergic neurons in vitro , we explored whether cells genetically modified to produce bFGF would improve the functional efficacy of dopaminergic neurons implanted into rats with experimental Parkinson 's disease .
	manualset3
136543	5	407029	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Since basic fibroblast growth factor ( bFGF ) enhances the survival and growth of dopaminergic neurons in vitro , we explored whether cells genetically modified to produce bFGF would improve the functional efficacy of dopaminergic neurons implanted into rats with experimental Parkinson 's disease .
	manualset3
136544	6	407029	5	NULL	NULL	0	NULL	bFGF 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Since basic fibroblast growth factor ( bFGF ) enhances the survival and growth of dopaminergic neurons in vitro , we explored whether cells genetically modified to produce bFGF would improve the functional efficacy of dopaminergic neurons implanted into rats with experimental Parkinson 's disease .
	manualset3
136545	7	407029	5	NULL	NULL	NULL	NULL	functional efficacy	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Since basic fibroblast growth factor ( bFGF ) enhances the survival and growth of dopaminergic neurons in vitro , we explored whether cells genetically modified to produce bFGF would improve the functional efficacy of dopaminergic neurons implanted into rats with experimental Parkinson 's disease .
	manualset3
136546	8	407029	5	NULL	NULL	0	NULL	dopaminergic neurons 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Since basic fibroblast growth factor ( bFGF ) enhances the survival and growth of dopaminergic neurons in vitro , we explored whether cells genetically modified to produce bFGF would improve the functional efficacy of dopaminergic neurons implanted into rats with experimental Parkinson 's disease .
	manualset3
136547	9	407029	5	NULL	NULL	0	NULL	rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Since basic fibroblast growth factor ( bFGF ) enhances the survival and growth of dopaminergic neurons in vitro , we explored whether cells genetically modified to produce bFGF would improve the functional efficacy of dopaminergic neurons implanted into rats with experimental Parkinson 's disease .
	manualset3
136548	10	407029	5	NULL	NULL	0	NULL	Parkinson 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Since basic fibroblast growth factor ( bFGF ) enhances the survival and growth of dopaminergic neurons in vitro , we explored whether cells genetically modified to produce bFGF would improve the functional efficacy of dopaminergic neurons implanted into rats with experimental Parkinson 's disease .
	manualset3
136549	1	407030	5	NULL	NULL	0	NULL	novel taxol-induced vimentin phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel taxol-induced vimentin phosphorylation and stabilization revealed by studies on stable microtubules and vimentin intermediate filaments .
	manualset3
136550	2	407030	5	NULL	NULL	0	NULL	stabilization 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel taxol-induced vimentin phosphorylation and stabilization revealed by studies on stable microtubules and vimentin intermediate filaments .
	manualset3
136551	3	407030	5	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel taxol-induced vimentin phosphorylation and stabilization revealed by studies on stable microtubules and vimentin intermediate filaments .
	manualset3
136552	4	407030	5	NULL	NULL	0	NULL	stable microtubules	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel taxol-induced vimentin phosphorylation and stabilization revealed by studies on stable microtubules and vimentin intermediate filaments .
	manualset3
136553	5	407030	5	NULL	NULL	0	NULL	vimentin intermediate filaments 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel taxol-induced vimentin phosphorylation and stabilization revealed by studies on stable microtubules and vimentin intermediate filaments .
	manualset3
136684	1	407031	5	NULL	NULL	0	NULL	age 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Since both age of menarche and age of marriage have increased , fertility among females age 15-19 may be expected to decrease in the future if this pattern continues .
	manualset3
136685	2	407031	5	NULL	NULL	0	NULL	menarche 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since both age of menarche and age of marriage have increased , fertility among females age 15-19 may be expected to decrease in the future if this pattern continues .
	manualset3
136687	3	407031	5	NULL	NULL	0	NULL	age 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Since both age of menarche and age of marriage have increased , fertility among females age 15-19 may be expected to decrease in the future if this pattern continues .
	manualset3
136691	4	407031	5	NULL	NULL	0	NULL	marriage 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since both age of menarche and age of marriage have increased , fertility among females age 15-19 may be expected to decrease in the future if this pattern continues .
	manualset3
136709	5	407031	5	NULL	NULL	0	NULL	fertility 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since both age of menarche and age of marriage have increased , fertility among females age 15-19 may be expected to decrease in the future if this pattern continues .
	manualset3
136710	6	407031	5	NULL	NULL	0	NULL	females 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since both age of menarche and age of marriage have increased , fertility among females age 15-19 may be expected to decrease in the future if this pattern continues .
	manualset3
136711	7	407031	5	NULL	NULL	0	NULL	age 15-19 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Since both age of menarche and age of marriage have increased , fertility among females age 15-19 may be expected to decrease in the future if this pattern continues .
	manualset3
136712	8	407031	5	NULL	NULL	0	NULL	decrease 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since both age of menarche and age of marriage have increased , fertility among females age 15-19 may be expected to decrease in the future if this pattern continues .
	manualset3
136713	9	407031	5	NULL	NULL	0	NULL	future 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Since both age of menarche and age of marriage have increased , fertility among females age 15-19 may be expected to decrease in the future if this pattern continues .
	manualset3
136714	10	407031	5	NULL	NULL	0	NULL	pattern 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since both age of menarche and age of marriage have increased , fertility among females age 15-19 may be expected to decrease in the future if this pattern continues .
	manualset3
136715	1	407032	5	NULL	NULL	0	NULL	health care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Since both the health care and airlines industries deal with a service rather than a product , the customer experience depends on the people who deliver that experience .
	manualset3
136716	2	407032	5	NULL	NULL	0	NULL	airlines industries 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Since both the health care and airlines industries deal with a service rather than a product , the customer experience depends on the people who deliver that experience .
	manualset3
136717	3	407032	5	NULL	NULL	0	NULL	service 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since both the health care and airlines industries deal with a service rather than a product , the customer experience depends on the people who deliver that experience .
	manualset3
136718	4	407032	5	NULL	NULL	0	NULL	product 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since both the health care and airlines industries deal with a service rather than a product , the customer experience depends on the people who deliver that experience .
	manualset3
136719	5	407032	5	NULL	NULL	0	NULL	customer experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since both the health care and airlines industries deal with a service rather than a product , the customer experience depends on the people who deliver that experience .
	manualset3
136720	6	407032	5	NULL	NULL	0	NULL	people 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since both the health care and airlines industries deal with a service rather than a product , the customer experience depends on the people who deliver that experience .
	manualset3
136721	7	407032	5	NULL	NULL	0	NULL	experience 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since both the health care and airlines industries deal with a service rather than a product , the customer experience depends on the people who deliver that experience .
	manualset3
136722	1	407033	5	NULL	NULL	0	NULL	 epsilon-proteobacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Since epsilon-proteobacteria closely related to these two organisms are important in many habitats , such as hydrothermal vents , oxic-sulfidic interfaces , or oilfields , these results suggest that autotrophic CO ( 2 ) fixation via the reductive tricarboxylic acid cycle might be more important than previously considered .
	manualset3
136723	2	407033	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Since epsilon-proteobacteria closely related to these two organisms are important in many habitats , such as hydrothermal vents , oxic-sulfidic interfaces , or oilfields , these results suggest that autotrophic CO ( 2 ) fixation via the reductive tricarboxylic acid cycle might be more important than previously considered .
	manualset3
136724	3	407033	5	NULL	NULL	NULL	NULL	organisms 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Since epsilon-proteobacteria closely related to these two organisms are important in many habitats , such as hydrothermal vents , oxic-sulfidic interfaces , or oilfields , these results suggest that autotrophic CO ( 2 ) fixation via the reductive tricarboxylic acid cycle might be more important than previously considered .
	manualset3
136725	4	407033	5	NULL	NULL	0	NULL	habitats 	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Since epsilon-proteobacteria closely related to these two organisms are important in many habitats , such as hydrothermal vents , oxic-sulfidic interfaces , or oilfields , these results suggest that autotrophic CO ( 2 ) fixation via the reductive tricarboxylic acid cycle might be more important than previously considered .
	manualset3
136726	5	407033	5	NULL	NULL	NULL	NULL	hydrothermal vents	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Since epsilon-proteobacteria closely related to these two organisms are important in many habitats , such as hydrothermal vents , oxic-sulfidic interfaces , or oilfields , these results suggest that autotrophic CO ( 2 ) fixation via the reductive tricarboxylic acid cycle might be more important than previously considered .
	manualset3
136727	6	407033	5	NULL	NULL	0	NULL	oxic-sulfidic interfaces	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Since epsilon-proteobacteria closely related to these two organisms are important in many habitats , such as hydrothermal vents , oxic-sulfidic interfaces , or oilfields , these results suggest that autotrophic CO ( 2 ) fixation via the reductive tricarboxylic acid cycle might be more important than previously considered .
	manualset3
136728	7	407033	5	NULL	NULL	0	NULL	oilfields 	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Since epsilon-proteobacteria closely related to these two organisms are important in many habitats , such as hydrothermal vents , oxic-sulfidic interfaces , or oilfields , these results suggest that autotrophic CO ( 2 ) fixation via the reductive tricarboxylic acid cycle might be more important than previously considered .
	manualset3
136729	8	407033	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Since epsilon-proteobacteria closely related to these two organisms are important in many habitats , such as hydrothermal vents , oxic-sulfidic interfaces , or oilfields , these results suggest that autotrophic CO ( 2 ) fixation via the reductive tricarboxylic acid cycle might be more important than previously considered .
	manualset3
136730	9	407033	5	NULL	NULL	0	NULL	autotrophic CO ( 2 ) fixation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since epsilon-proteobacteria closely related to these two organisms are important in many habitats , such as hydrothermal vents , oxic-sulfidic interfaces , or oilfields , these results suggest that autotrophic CO ( 2 ) fixation via the reductive tricarboxylic acid cycle might be more important than previously considered .
	manualset3
136731	10	407033	5	NULL	NULL	0	NULL	reductive tricarboxylic acid cycle	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since epsilon-proteobacteria closely related to these two organisms are important in many habitats , such as hydrothermal vents , oxic-sulfidic interfaces , or oilfields , these results suggest that autotrophic CO ( 2 ) fixation via the reductive tricarboxylic acid cycle might be more important than previously considered .
	manualset3
136732	1	407034	5	NULL	NULL	0	NULL	expression profiling methods 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since expression profiling methods have been available in a high throughput fashion , the implication of these technologies in the field of biotechnology has increased dramatically .
	manualset3
136733	2	407034	5	NULL	NULL	0	NULL	high throughput fashion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since expression profiling methods have been available in a high throughput fashion , the implication of these technologies in the field of biotechnology has increased dramatically .
	manualset3
136734	3	407034	5	NULL	NULL	0	NULL	implication 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since expression profiling methods have been available in a high throughput fashion , the implication of these technologies in the field of biotechnology has increased dramatically .
	manualset3
136735	4	407034	5	NULL	NULL	0	NULL	technologies 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since expression profiling methods have been available in a high throughput fashion , the implication of these technologies in the field of biotechnology has increased dramatically .
	manualset3
136736	5	407034	5	NULL	NULL	0	NULL	field 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since expression profiling methods have been available in a high throughput fashion , the implication of these technologies in the field of biotechnology has increased dramatically .
	manualset3
136737	6	407034	5	NULL	NULL	0	NULL	biotechnology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since expression profiling methods have been available in a high throughput fashion , the implication of these technologies in the field of biotechnology has increased dramatically .
	manualset3
136738	1	407035	5	NULL	NULL	0	NULL	family planning	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Since family planning is an integral part of development , continued U.S. assistance in the field of population and family planning is necessary .
	manualset3
136739	2	407035	5	NULL	NULL	0	NULL	integral part 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since family planning is an integral part of development , continued U.S. assistance in the field of population and family planning is necessary .
	manualset3
136740	3	407035	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since family planning is an integral part of development , continued U.S. assistance in the field of population and family planning is necessary .
	manualset3
136741	4	407035	5	NULL	NULL	0	NULL	continued U.S. assistance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since family planning is an integral part of development , continued U.S. assistance in the field of population and family planning is necessary .
	manualset3
136742	5	407035	5	NULL	NULL	0	NULL	field 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since family planning is an integral part of development , continued U.S. assistance in the field of population and family planning is necessary .
	manualset3
136743	6	407035	5	NULL	NULL	0	NULL	population and family planning 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Since family planning is an integral part of development , continued U.S. assistance in the field of population and family planning is necessary .
	manualset3
136744	1	407036	5	NULL	NULL	0	NULL	gangliosides 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Since gangliosides are poor immunogens and T-cell independent antigens , an adjuvant ( monophosphoryl lipid A ( MPL ) , a non-toxic lipid A of Salmonella ) , directed against B-cells , was employed .
	manualset3
136745	2	407036	5	NULL	NULL	0	NULL	immunogens 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Since gangliosides are poor immunogens and T-cell independent antigens , an adjuvant ( monophosphoryl lipid A ( MPL ) , a non-toxic lipid A of Salmonella ) , directed against B-cells , was employed .
	manualset3
136746	3	407036	5	NULL	NULL	0	NULL	 T-cell independent antigens	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Since gangliosides are poor immunogens and T-cell independent antigens , an adjuvant ( monophosphoryl lipid A ( MPL ) , a non-toxic lipid A of Salmonella ) , directed against B-cells , was employed .
	manualset3
136747	4	407036	5	NULL	NULL	0	NULL	adjuvant 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Since gangliosides are poor immunogens and T-cell independent antigens , an adjuvant ( monophosphoryl lipid A ( MPL ) , a non-toxic lipid A of Salmonella ) , directed against B-cells , was employed .
	manualset3
136748	5	407036	5	NULL	NULL	0	NULL	monophosphoryl lipid A ( MPL ) , a non-toxic lipid A of Salmonella	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Since gangliosides are poor immunogens and T-cell independent antigens , an adjuvant ( monophosphoryl lipid A ( MPL ) , a non-toxic lipid A of Salmonella ) , directed against B-cells , was employed .
	manualset3
136749	6	407036	5	NULL	NULL	0	NULL	B-cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Since gangliosides are poor immunogens and T-cell independent antigens , an adjuvant ( monophosphoryl lipid A ( MPL ) , a non-toxic lipid A of Salmonella ) , directed against B-cells , was employed .
	manualset3
136750	1	407037	5	NULL	NULL	0	NULL	vitamin D3	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Since it is known that vitamin D3 up regulates and glucocorticoid down regulates transcription of the osteocalcin gene , the endocrine response evoked by tail suspension may have aggravated the disuse atrophy caused by skeletal unloading in this study .
	manualset3
136751	2	407037	5	NULL	NULL	0	NULL	glucocorticoid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Since it is known that vitamin D3 up regulates and glucocorticoid down regulates transcription of the osteocalcin gene , the endocrine response evoked by tail suspension may have aggravated the disuse atrophy caused by skeletal unloading in this study .
	manualset3
136752	3	407037	5	NULL	NULL	0	NULL	transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since it is known that vitamin D3 up regulates and glucocorticoid down regulates transcription of the osteocalcin gene , the endocrine response evoked by tail suspension may have aggravated the disuse atrophy caused by skeletal unloading in this study .
	manualset3
136753	4	407037	5	NULL	NULL	0	NULL	osteocalcin gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Since it is known that vitamin D3 up regulates and glucocorticoid down regulates transcription of the osteocalcin gene , the endocrine response evoked by tail suspension may have aggravated the disuse atrophy caused by skeletal unloading in this study .
	manualset3
136754	5	407037	5	NULL	NULL	0	NULL	endocrine response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since it is known that vitamin D3 up regulates and glucocorticoid down regulates transcription of the osteocalcin gene , the endocrine response evoked by tail suspension may have aggravated the disuse atrophy caused by skeletal unloading in this study .
	manualset3
136755	6	407037	5	NULL	NULL	0	NULL	tail suspension	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since it is known that vitamin D3 up regulates and glucocorticoid down regulates transcription of the osteocalcin gene , the endocrine response evoked by tail suspension may have aggravated the disuse atrophy caused by skeletal unloading in this study .
	manualset3
136756	7	407037	5	NULL	NULL	0	NULL	disuse atrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since it is known that vitamin D3 up regulates and glucocorticoid down regulates transcription of the osteocalcin gene , the endocrine response evoked by tail suspension may have aggravated the disuse atrophy caused by skeletal unloading in this study .
	manualset3
136757	8	407037	5	NULL	NULL	0	NULL	skeletal unloading	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since it is known that vitamin D3 up regulates and glucocorticoid down regulates transcription of the osteocalcin gene , the endocrine response evoked by tail suspension may have aggravated the disuse atrophy caused by skeletal unloading in this study .
	manualset3
136758	9	407037	5	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since it is known that vitamin D3 up regulates and glucocorticoid down regulates transcription of the osteocalcin gene , the endocrine response evoked by tail suspension may have aggravated the disuse atrophy caused by skeletal unloading in this study .
	manualset3
136759	1	407038	5	NULL	NULL	0	NULL	hexamer	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Since it was documented that hexamer is very potent in activating complement , it is suggested that its production in humans must be under strict control , and that it is produced in special conditions , when strong activation of complement is absolutely needed .
	manualset3
136760	2	407038	5	NULL	NULL	0	NULL	complement	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since it was documented that hexamer is very potent in activating complement , it is suggested that its production in humans must be under strict control , and that it is produced in special conditions , when strong activation of complement is absolutely needed .
	manualset3
136761	3	407038	5	NULL	NULL	0	NULL	production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since it was documented that hexamer is very potent in activating complement , it is suggested that its production in humans must be under strict control , and that it is produced in special conditions , when strong activation of complement is absolutely needed .
	manualset3
136762	4	407038	5	NULL	NULL	0	NULL	humans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Since it was documented that hexamer is very potent in activating complement , it is suggested that its production in humans must be under strict control , and that it is produced in special conditions , when strong activation of complement is absolutely needed .
	manualset3
136763	5	407038	5	NULL	NULL	0	NULL	strict control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since it was documented that hexamer is very potent in activating complement , it is suggested that its production in humans must be under strict control , and that it is produced in special conditions , when strong activation of complement is absolutely needed .
	manualset3
136764	6	407038	5	NULL	NULL	0	NULL	special conditions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since it was documented that hexamer is very potent in activating complement , it is suggested that its production in humans must be under strict control , and that it is produced in special conditions , when strong activation of complement is absolutely needed .
	manualset3
136765	7	407038	5	NULL	NULL	NULL	NULL	strong activation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Since it was documented that hexamer is very potent in activating complement , it is suggested that its production in humans must be under strict control , and that it is produced in special conditions , when strong activation of complement is absolutely needed .
	manualset3
136766	8	407038	5	NULL	NULL	0	NULL	complement	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since it was documented that hexamer is very potent in activating complement , it is suggested that its production in humans must be under strict control , and that it is produced in special conditions , when strong activation of complement is absolutely needed .
	manualset3
136767	1	407039	5	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of adipocytokines are increased in obesity causing low-level chronic inflammation associated with an increased risk of tumors .
	manualset3
136768	2	407039	5	NULL	NULL	0	NULL	adipocytokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of adipocytokines are increased in obesity causing low-level chronic inflammation associated with an increased risk of tumors .
	manualset3
136769	3	407039	5	NULL	NULL	0	NULL	obesity	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of adipocytokines are increased in obesity causing low-level chronic inflammation associated with an increased risk of tumors .
	manualset3
136770	4	407039	5	NULL	NULL	0	NULL	 low-level chronic inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of adipocytokines are increased in obesity causing low-level chronic inflammation associated with an increased risk of tumors .
	manualset3
136771	5	407039	5	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of adipocytokines are increased in obesity causing low-level chronic inflammation associated with an increased risk of tumors .
	manualset3
136772	6	407039	5	NULL	NULL	0	NULL	tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of adipocytokines are increased in obesity causing low-level chronic inflammation associated with an increased risk of tumors .
	manualset3
136773	1	407040	5	NULL	NULL	0	NULL	discovery	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since its discovery , serotonin ( 5-hydroxytryptamine = 5-HT ) has become a major player on the neurotransmitter `` stage '' .
	manualset3
136774	2	407040	5	NULL	NULL	0	NULL	serotonin ( 5-hydroxytryptamine = 5-HT )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Since its discovery , serotonin ( 5-hydroxytryptamine = 5-HT ) has become a major player on the neurotransmitter `` stage '' .
	manualset3
136775	3	407040	5	NULL	NULL	0	NULL	major player	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since its discovery , serotonin ( 5-hydroxytryptamine = 5-HT ) has become a major player on the neurotransmitter `` stage '' .
	manualset3
136776	4	407040	5	NULL	NULL	0	NULL	neurotransmitter `` stage ''	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since its discovery , serotonin ( 5-hydroxytryptamine = 5-HT ) has become a major player on the neurotransmitter `` stage '' .
	manualset3
136777	1	407041	5	NULL	NULL	0	NULL	1921	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Since its founding in 1921 , the mission of the Maternal and Child Health ( MCH ) Section of the American Public Health Association ( APHA ) has been to develop innovative and creative approaches to addressing the health needs of mothers , children , and families .
	manualset3
136778	2	407041	5	NULL	NULL	0	NULL	mission	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since its founding in 1921 , the mission of the Maternal and Child Health ( MCH ) Section of the American Public Health Association ( APHA ) has been to develop innovative and creative approaches to addressing the health needs of mothers , children , and families .
	manualset3
136779	3	407041	5	NULL	NULL	NULL	NULL	Maternal and Child Health ( MCH ) Section	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Since its founding in 1921 , the mission of the Maternal and Child Health ( MCH ) Section of the American Public Health Association ( APHA ) has been to develop innovative and creative approaches to addressing the health needs of mothers , children , and families .
	manualset3
136780	4	407041	5	NULL	NULL	0	NULL	American Public Health Association ( APHA ) 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since its founding in 1921 , the mission of the Maternal and Child Health ( MCH ) Section of the American Public Health Association ( APHA ) has been to develop innovative and creative approaches to addressing the health needs of mothers , children , and families .
	manualset3
136781	5	407041	5	NULL	NULL	0	NULL	innovative approaches	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since its founding in 1921 , the mission of the Maternal and Child Health ( MCH ) Section of the American Public Health Association ( APHA ) has been to develop innovative and creative approaches to addressing the health needs of mothers , children , and families .
	manualset3
136782	6	407041	5	NULL	NULL	0	NULL	creative approaches	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since its founding in 1921 , the mission of the Maternal and Child Health ( MCH ) Section of the American Public Health Association ( APHA ) has been to develop innovative and creative approaches to addressing the health needs of mothers , children , and families .
	manualset3
136783	7	407041	5	NULL	NULL	NULL	NULL	health needs	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Since its founding in 1921 , the mission of the Maternal and Child Health ( MCH ) Section of the American Public Health Association ( APHA ) has been to develop innovative and creative approaches to addressing the health needs of mothers , children , and families .
	manualset3
136784	8	407041	5	NULL	NULL	0	NULL	mothers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since its founding in 1921 , the mission of the Maternal and Child Health ( MCH ) Section of the American Public Health Association ( APHA ) has been to develop innovative and creative approaches to addressing the health needs of mothers , children , and families .
	manualset3
136785	9	407041	5	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since its founding in 1921 , the mission of the Maternal and Child Health ( MCH ) Section of the American Public Health Association ( APHA ) has been to develop innovative and creative approaches to addressing the health needs of mothers , children , and families .
	manualset3
136786	10	407041	5	NULL	NULL	0	NULL	families	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since its founding in 1921 , the mission of the Maternal and Child Health ( MCH ) Section of the American Public Health Association ( APHA ) has been to develop innovative and creative approaches to addressing the health needs of mothers , children , and families .
	manualset3
136787	1	407042	5	NULL	NULL	0	NULL	inception	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since its inception , psychoanalysts and analytical psychologists have used the reductionistic methods of science to explain both human development and analytic practice .
	manualset3
136788	2	407042	5	NULL	NULL	0	NULL	psychoanalysts	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since its inception , psychoanalysts and analytical psychologists have used the reductionistic methods of science to explain both human development and analytic practice .
	manualset3
136789	3	407042	5	NULL	NULL	0	NULL	analytical psychologists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since its inception , psychoanalysts and analytical psychologists have used the reductionistic methods of science to explain both human development and analytic practice .
	manualset3
136790	4	407042	5	NULL	NULL	0	NULL	reductionistic methods	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Since its inception , psychoanalysts and analytical psychologists have used the reductionistic methods of science to explain both human development and analytic practice .
	manualset3
136791	5	407042	5	NULL	NULL	0	NULL	science	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since its inception , psychoanalysts and analytical psychologists have used the reductionistic methods of science to explain both human development and analytic practice .
	manualset3
136792	6	407042	5	NULL	NULL	0	NULL	human development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since its inception , psychoanalysts and analytical psychologists have used the reductionistic methods of science to explain both human development and analytic practice .
	manualset3
136793	7	407042	5	NULL	NULL	0	NULL	analytic practice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since its inception , psychoanalysts and analytical psychologists have used the reductionistic methods of science to explain both human development and analytic practice .
	manualset3
136794	1	407043	5	NULL	NULL	0	NULL	therapies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Since many of these therapies have targeted key pathways in asthma pathology these studies provide information on patient stratification and asthma pathology .
	manualset3
136795	2	407043	5	NULL	NULL	0	NULL	key pathways 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since many of these therapies have targeted key pathways in asthma pathology these studies provide information on patient stratification and asthma pathology .
	manualset3
136796	3	407043	5	NULL	NULL	0	NULL	asthma pathology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since many of these therapies have targeted key pathways in asthma pathology these studies provide information on patient stratification and asthma pathology .
	manualset3
136797	4	407043	5	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since many of these therapies have targeted key pathways in asthma pathology these studies provide information on patient stratification and asthma pathology .
	manualset3
136798	5	407043	5	NULL	NULL	0	NULL	information	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since many of these therapies have targeted key pathways in asthma pathology these studies provide information on patient stratification and asthma pathology .
	manualset3
136799	6	407043	5	NULL	NULL	0	NULL	patient stratification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since many of these therapies have targeted key pathways in asthma pathology these studies provide information on patient stratification and asthma pathology .
	manualset3
136800	7	407043	5	NULL	NULL	0	NULL	asthma pathology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since many of these therapies have targeted key pathways in asthma pathology these studies provide information on patient stratification and asthma pathology .
	manualset3
136801	1	407044	5	NULL	NULL	0	NULL	microalbuminuria	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since microalbuminuria ( albumin excretion rate ) 30 mg/day ) represents an incipient stage of diabetic nephropathy , we decided to investigate whether incipient renal changes correlate with early diastolic cardiac dysfunction , known to preceed systolic dysfunction .
	manualset3
136802	2	407044	5	NULL	NULL	0	NULL	albumin excretion rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since microalbuminuria ( albumin excretion rate ) 30 mg/day ) represents an incipient stage of diabetic nephropathy , we decided to investigate whether incipient renal changes correlate with early diastolic cardiac dysfunction , known to preceed systolic dysfunction .
	manualset3
136803	3	407044	5	NULL	NULL	0	NULL	 30 mg/day 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Since microalbuminuria ( albumin excretion rate ) 30 mg/day ) represents an incipient stage of diabetic nephropathy , we decided to investigate whether incipient renal changes correlate with early diastolic cardiac dysfunction , known to preceed systolic dysfunction .
	manualset3
136804	4	407044	5	NULL	NULL	0	NULL	incipient stage	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Since microalbuminuria ( albumin excretion rate ) 30 mg/day ) represents an incipient stage of diabetic nephropathy , we decided to investigate whether incipient renal changes correlate with early diastolic cardiac dysfunction , known to preceed systolic dysfunction .
	manualset3
136805	5	407044	5	NULL	NULL	0	NULL	diabetic nephropathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Since microalbuminuria ( albumin excretion rate ) 30 mg/day ) represents an incipient stage of diabetic nephropathy , we decided to investigate whether incipient renal changes correlate with early diastolic cardiac dysfunction , known to preceed systolic dysfunction .
	manualset3
136806	6	407044	5	NULL	NULL	0	NULL	investigate	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since microalbuminuria ( albumin excretion rate ) 30 mg/day ) represents an incipient stage of diabetic nephropathy , we decided to investigate whether incipient renal changes correlate with early diastolic cardiac dysfunction , known to preceed systolic dysfunction .
	manualset3
136807	7	407044	5	NULL	NULL	0	NULL	incipient renal changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since microalbuminuria ( albumin excretion rate ) 30 mg/day ) represents an incipient stage of diabetic nephropathy , we decided to investigate whether incipient renal changes correlate with early diastolic cardiac dysfunction , known to preceed systolic dysfunction .
	manualset3
136808	8	407044	5	NULL	NULL	0	NULL	early diastolic cardiac dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since microalbuminuria ( albumin excretion rate ) 30 mg/day ) represents an incipient stage of diabetic nephropathy , we decided to investigate whether incipient renal changes correlate with early diastolic cardiac dysfunction , known to preceed systolic dysfunction .
	manualset3
136809	9	407044	5	NULL	NULL	0	NULL	systolic dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since microalbuminuria ( albumin excretion rate ) 30 mg/day ) represents an incipient stage of diabetic nephropathy , we decided to investigate whether incipient renal changes correlate with early diastolic cardiac dysfunction , known to preceed systolic dysfunction .
	manualset3
136810	1	407045	5	NULL	NULL	0	NULL	mutant	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Since neither mutant would complement the ftsH defect produced in the absence of arabinose , we conclude that the protease function of FtsH is required for bacterial growth .
	manualset3
136812	3	407045	5	NULL	NULL	0	NULL	ftsH defect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since neither mutant would complement the ftsH defect produced in the absence of arabinose , we conclude that the protease function of FtsH is required for bacterial growth .
	manualset3
136813	4	407045	5	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since neither mutant would complement the ftsH defect produced in the absence of arabinose , we conclude that the protease function of FtsH is required for bacterial growth .
	manualset3
136814	5	407045	5	NULL	NULL	0	NULL	arabinose	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Since neither mutant would complement the ftsH defect produced in the absence of arabinose , we conclude that the protease function of FtsH is required for bacterial growth .
	manualset3
136815	6	407045	5	NULL	NULL	0	NULL	protease function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since neither mutant would complement the ftsH defect produced in the absence of arabinose , we conclude that the protease function of FtsH is required for bacterial growth .
	manualset3
136816	7	407045	5	NULL	NULL	0	NULL	FtsH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Since neither mutant would complement the ftsH defect produced in the absence of arabinose , we conclude that the protease function of FtsH is required for bacterial growth .
	manualset3
136817	8	407045	5	NULL	NULL	0	NULL	bacterial growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since neither mutant would complement the ftsH defect produced in the absence of arabinose , we conclude that the protease function of FtsH is required for bacterial growth .
	manualset3
136818	1	407046	5	NULL	NULL	0	NULL	donor HLA-specific gamma delta T cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Since no donor HLA-specific gamma delta T cells have been detected , other ligands , such as heat shock proteins , may be involved .
	manualset3
136819	2	407046	5	NULL	NULL	0	NULL	ligands	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Since no donor HLA-specific gamma delta T cells have been detected , other ligands , such as heat shock proteins , may be involved .
	manualset3
136820	3	407046	5	NULL	NULL	0	NULL	heat shock proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since no donor HLA-specific gamma delta T cells have been detected , other ligands , such as heat shock proteins , may be involved .
	manualset3
136821	1	407047	5	NULL	NULL	0	NULL	androgen responsive elements	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Since no obvious androgen responsive elements were included in the promoter region , we suggest that the stimulation of the reporter construct has to be mediated indirectly by androgen-dependent transcription factor ( s ) .
	manualset3
136822	2	407047	5	NULL	NULL	0	NULL	promoter region 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Since no obvious androgen responsive elements were included in the promoter region , we suggest that the stimulation of the reporter construct has to be mediated indirectly by androgen-dependent transcription factor ( s ) .
	manualset3
136823	3	407047	5	NULL	NULL	0	NULL	stimulation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since no obvious androgen responsive elements were included in the promoter region , we suggest that the stimulation of the reporter construct has to be mediated indirectly by androgen-dependent transcription factor ( s ) .
	manualset3
136824	4	407047	5	NULL	NULL	0	NULL	reporter construct	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Since no obvious androgen responsive elements were included in the promoter region , we suggest that the stimulation of the reporter construct has to be mediated indirectly by androgen-dependent transcription factor ( s ) .
	manualset3
136825	5	407047	5	NULL	NULL	0	NULL	androgen-dependent transcription factor ( s )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since no obvious androgen responsive elements were included in the promoter region , we suggest that the stimulation of the reporter construct has to be mediated indirectly by androgen-dependent transcription factor ( s ) .
	manualset3
136826	1	407048	5	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of challenges need to be addressed to deliver pediatric cardiac intensive care in the developing world .
	manualset3
136827	2	407048	5	NULL	NULL	0	NULL	challenges	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of challenges need to be addressed to deliver pediatric cardiac intensive care in the developing world .
	manualset3
136828	3	407048	5	NULL	NULL	0	NULL	pediatric cardiac intensive care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of challenges need to be addressed to deliver pediatric cardiac intensive care in the developing world .
	manualset3
136829	4	407048	5	NULL	NULL	0	NULL	developing world	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of challenges need to be addressed to deliver pediatric cardiac intensive care in the developing world .
	manualset3
136830	1	407049	5	NULL	NULL	NULL	NULL	potential therapeutic indications	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Since numerous potential therapeutic indications have been identified for BLyS and other BLyS-derived products , large quantities of the protein are needed to further basic research and clinical trials .
	manualset3
136831	2	407049	5	NULL	NULL	NULL	NULL	BLyS	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Since numerous potential therapeutic indications have been identified for BLyS and other BLyS-derived products , large quantities of the protein are needed to further basic research and clinical trials .
	manualset3
136832	3	407049	5	NULL	NULL	0	NULL	BLyS-derived products	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since numerous potential therapeutic indications have been identified for BLyS and other BLyS-derived products , large quantities of the protein are needed to further basic research and clinical trials .
	manualset3
136833	4	407049	5	NULL	NULL	0	NULL	large quantities	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since numerous potential therapeutic indications have been identified for BLyS and other BLyS-derived products , large quantities of the protein are needed to further basic research and clinical trials .
	manualset3
136834	5	407049	5	NULL	NULL	0	NULL	protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Since numerous potential therapeutic indications have been identified for BLyS and other BLyS-derived products , large quantities of the protein are needed to further basic research and clinical trials .
	manualset3
136835	6	407049	5	NULL	NULL	0	NULL	basic research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since numerous potential therapeutic indications have been identified for BLyS and other BLyS-derived products , large quantities of the protein are needed to further basic research and clinical trials .
	manualset3
136836	7	407049	5	NULL	NULL	0	NULL	clinical trials	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since numerous potential therapeutic indications have been identified for BLyS and other BLyS-derived products , large quantities of the protein are needed to further basic research and clinical trials .
	manualset3
136837	1	407050	5	NULL	NULL	0	NULL	reports 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Since other reports have shown that RTN4-A inhibits neuronal outgrowth and restricts the plasticity of the central nervous system , we speculate that RTN3-A1 might play certain roles in the central nervous system .
	manualset3
136838	2	407050	5	NULL	NULL	0	NULL	RTN4-A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Since other reports have shown that RTN4-A inhibits neuronal outgrowth and restricts the plasticity of the central nervous system , we speculate that RTN3-A1 might play certain roles in the central nervous system .
	manualset3
136839	3	407050	5	NULL	NULL	0	NULL	neuronal outgrowth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since other reports have shown that RTN4-A inhibits neuronal outgrowth and restricts the plasticity of the central nervous system , we speculate that RTN3-A1 might play certain roles in the central nervous system .
	manualset3
136840	4	407050	5	NULL	NULL	0	NULL	plasticity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since other reports have shown that RTN4-A inhibits neuronal outgrowth and restricts the plasticity of the central nervous system , we speculate that RTN3-A1 might play certain roles in the central nervous system .
	manualset3
136841	5	407050	5	NULL	NULL	0	NULL	central nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Since other reports have shown that RTN4-A inhibits neuronal outgrowth and restricts the plasticity of the central nervous system , we speculate that RTN3-A1 might play certain roles in the central nervous system .
	manualset3
136842	6	407050	5	NULL	NULL	0	NULL	RTN3-A1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Since other reports have shown that RTN4-A inhibits neuronal outgrowth and restricts the plasticity of the central nervous system , we speculate that RTN3-A1 might play certain roles in the central nervous system .
	manualset3
136843	7	407050	5	NULL	NULL	0	NULL	roles 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since other reports have shown that RTN4-A inhibits neuronal outgrowth and restricts the plasticity of the central nervous system , we speculate that RTN3-A1 might play certain roles in the central nervous system .
	manualset3
136844	8	407050	5	NULL	NULL	0	NULL	central nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Since other reports have shown that RTN4-A inhibits neuronal outgrowth and restricts the plasticity of the central nervous system , we speculate that RTN3-A1 might play certain roles in the central nervous system .
	manualset3
136845	1	407051	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since our aim was to isolate and identify new progression markers of human cutaneous melanoma , we applied the differential hybridization technique , in which we compared the gene expression in two subsequent stages of this progression .
	manualset3
136846	2	407051	5	NULL	NULL	0	NULL	isolate 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since our aim was to isolate and identify new progression markers of human cutaneous melanoma , we applied the differential hybridization technique , in which we compared the gene expression in two subsequent stages of this progression .
	manualset3
136847	3	407051	5	NULL	NULL	0	NULL	identify 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since our aim was to isolate and identify new progression markers of human cutaneous melanoma , we applied the differential hybridization technique , in which we compared the gene expression in two subsequent stages of this progression .
	manualset3
136848	4	407051	5	NULL	NULL	0	NULL	progression markers	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since our aim was to isolate and identify new progression markers of human cutaneous melanoma , we applied the differential hybridization technique , in which we compared the gene expression in two subsequent stages of this progression .
	manualset3
136849	5	407051	5	NULL	NULL	0	NULL	human cutaneous melanoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Since our aim was to isolate and identify new progression markers of human cutaneous melanoma , we applied the differential hybridization technique , in which we compared the gene expression in two subsequent stages of this progression .
	manualset3
136850	6	407051	5	NULL	NULL	0	NULL	differential hybridization technique 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since our aim was to isolate and identify new progression markers of human cutaneous melanoma , we applied the differential hybridization technique , in which we compared the gene expression in two subsequent stages of this progression .
	manualset3
136851	7	407051	5	NULL	NULL	0	NULL	gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since our aim was to isolate and identify new progression markers of human cutaneous melanoma , we applied the differential hybridization technique , in which we compared the gene expression in two subsequent stages of this progression .
	manualset3
136852	8	407051	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Since our aim was to isolate and identify new progression markers of human cutaneous melanoma , we applied the differential hybridization technique , in which we compared the gene expression in two subsequent stages of this progression .
	manualset3
136853	9	407051	5	NULL	NULL	0	NULL	subsequent stages	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Since our aim was to isolate and identify new progression markers of human cutaneous melanoma , we applied the differential hybridization technique , in which we compared the gene expression in two subsequent stages of this progression .
	manualset3
136854	10	407051	5	NULL	NULL	0	NULL	progression 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since our aim was to isolate and identify new progression markers of human cutaneous melanoma , we applied the differential hybridization technique , in which we compared the gene expression in two subsequent stages of this progression .
	manualset3
136855	1	407052	5	NULL	NULL	0	NULL	polyploidization 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since polyploidization may be considered as a cellular response to higher functional requirement ( i.e. inflammation or regeneration ) a `` suspicious '' cervical smear with a polyploid DNA-distribution pattern may reverse to normal cervical epithelium after normal conditions are restored .
	manualset3
136856	2	407052	5	NULL	NULL	0	NULL	cellular response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since polyploidization may be considered as a cellular response to higher functional requirement ( i.e. inflammation or regeneration ) a `` suspicious '' cervical smear with a polyploid DNA-distribution pattern may reverse to normal cervical epithelium after normal conditions are restored .
	manualset3
136857	3	407052	5	NULL	NULL	0	NULL	higher functional requirement	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since polyploidization may be considered as a cellular response to higher functional requirement ( i.e. inflammation or regeneration ) a `` suspicious '' cervical smear with a polyploid DNA-distribution pattern may reverse to normal cervical epithelium after normal conditions are restored .
	manualset3
136858	4	407052	5	NULL	NULL	0	NULL	inflammation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since polyploidization may be considered as a cellular response to higher functional requirement ( i.e. inflammation or regeneration ) a `` suspicious '' cervical smear with a polyploid DNA-distribution pattern may reverse to normal cervical epithelium after normal conditions are restored .
	manualset3
136859	5	407052	5	NULL	NULL	0	NULL	regeneration 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since polyploidization may be considered as a cellular response to higher functional requirement ( i.e. inflammation or regeneration ) a `` suspicious '' cervical smear with a polyploid DNA-distribution pattern may reverse to normal cervical epithelium after normal conditions are restored .
	manualset3
136860	6	407052	5	NULL	NULL	0	NULL	cervical smear	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Since polyploidization may be considered as a cellular response to higher functional requirement ( i.e. inflammation or regeneration ) a `` suspicious '' cervical smear with a polyploid DNA-distribution pattern may reverse to normal cervical epithelium after normal conditions are restored .
	manualset3
136861	7	407052	5	NULL	NULL	0	NULL	polyploid DNA-distribution pattern	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since polyploidization may be considered as a cellular response to higher functional requirement ( i.e. inflammation or regeneration ) a `` suspicious '' cervical smear with a polyploid DNA-distribution pattern may reverse to normal cervical epithelium after normal conditions are restored .
	manualset3
136862	8	407052	5	NULL	NULL	0	NULL	cervical epithelium 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Since polyploidization may be considered as a cellular response to higher functional requirement ( i.e. inflammation or regeneration ) a `` suspicious '' cervical smear with a polyploid DNA-distribution pattern may reverse to normal cervical epithelium after normal conditions are restored .
	manualset3
136863	9	407052	5	NULL	NULL	0	NULL	normal conditions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since polyploidization may be considered as a cellular response to higher functional requirement ( i.e. inflammation or regeneration ) a `` suspicious '' cervical smear with a polyploid DNA-distribution pattern may reverse to normal cervical epithelium after normal conditions are restored .
	manualset3
136864	1	407053	5	NULL	NULL	0	NULL	pouchitis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since pouchitis occurs more frequently or even exclusively in ulcerative colitis patients it is assumed that pouchitis is a novel manifestation of inflammatory bowel disease .
	manualset3
136865	2	407053	5	NULL	NULL	0	NULL	ulcerative colitis patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since pouchitis occurs more frequently or even exclusively in ulcerative colitis patients it is assumed that pouchitis is a novel manifestation of inflammatory bowel disease .
	manualset3
136866	3	407053	5	NULL	NULL	0	NULL	pouchitis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since pouchitis occurs more frequently or even exclusively in ulcerative colitis patients it is assumed that pouchitis is a novel manifestation of inflammatory bowel disease .
	manualset3
136867	4	407053	5	NULL	NULL	NULL	NULL	novel manifestation 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Since pouchitis occurs more frequently or even exclusively in ulcerative colitis patients it is assumed that pouchitis is a novel manifestation of inflammatory bowel disease .
	manualset3
136868	5	407053	5	NULL	NULL	0	NULL	inflammatory bowel disease 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since pouchitis occurs more frequently or even exclusively in ulcerative colitis patients it is assumed that pouchitis is a novel manifestation of inflammatory bowel disease .
	manualset3
136869	1	407054	5	NULL	NULL	0	NULL	pregnant women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since pregnant women may be exposed to untoward levels of Al compounds under certain conditions , we have examined the long-term effects of treating the pregnant mouse with intraperitoneal or oral aluminium sulphate on brain biochemistry and behavior of the offspring .
	manualset3
136870	2	407054	5	NULL	NULL	0	NULL	untoward levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since pregnant women may be exposed to untoward levels of Al compounds under certain conditions , we have examined the long-term effects of treating the pregnant mouse with intraperitoneal or oral aluminium sulphate on brain biochemistry and behavior of the offspring .
	manualset3
136871	3	407054	5	NULL	NULL	0	NULL	Al compounds	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Since pregnant women may be exposed to untoward levels of Al compounds under certain conditions , we have examined the long-term effects of treating the pregnant mouse with intraperitoneal or oral aluminium sulphate on brain biochemistry and behavior of the offspring .
	manualset3
136872	4	407054	5	NULL	NULL	0	NULL	conditions 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since pregnant women may be exposed to untoward levels of Al compounds under certain conditions , we have examined the long-term effects of treating the pregnant mouse with intraperitoneal or oral aluminium sulphate on brain biochemistry and behavior of the offspring .
	manualset3
136873	5	407054	5	NULL	NULL	0	NULL	long-term effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since pregnant women may be exposed to untoward levels of Al compounds under certain conditions , we have examined the long-term effects of treating the pregnant mouse with intraperitoneal or oral aluminium sulphate on brain biochemistry and behavior of the offspring .
	manualset3
136874	6	407054	5	NULL	NULL	0	NULL	pregnant mouse	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Since pregnant women may be exposed to untoward levels of Al compounds under certain conditions , we have examined the long-term effects of treating the pregnant mouse with intraperitoneal or oral aluminium sulphate on brain biochemistry and behavior of the offspring .
	manualset3
136875	7	407054	5	NULL	NULL	0	NULL	intraperitoneal or oral aluminium sulphate	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Since pregnant women may be exposed to untoward levels of Al compounds under certain conditions , we have examined the long-term effects of treating the pregnant mouse with intraperitoneal or oral aluminium sulphate on brain biochemistry and behavior of the offspring .
	manualset3
136876	8	407054	5	NULL	NULL	0	NULL	brain biochemistry	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since pregnant women may be exposed to untoward levels of Al compounds under certain conditions , we have examined the long-term effects of treating the pregnant mouse with intraperitoneal or oral aluminium sulphate on brain biochemistry and behavior of the offspring .
	manualset3
136877	9	407054	5	NULL	NULL	0	NULL	behavior 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since pregnant women may be exposed to untoward levels of Al compounds under certain conditions , we have examined the long-term effects of treating the pregnant mouse with intraperitoneal or oral aluminium sulphate on brain biochemistry and behavior of the offspring .
	manualset3
136878	10	407054	5	NULL	NULL	0	NULL	offspring 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Since pregnant women may be exposed to untoward levels of Al compounds under certain conditions , we have examined the long-term effects of treating the pregnant mouse with intraperitoneal or oral aluminium sulphate on brain biochemistry and behavior of the offspring .
	manualset3
136879	1	407055	5	NULL	NULL	0	NULL	 prenatal counselling 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Since prenatal counselling is now possible , the recognition of this severe familial under-diagnosed disease is of the upmost importance .
	manualset3
136880	2	407055	5	NULL	NULL	0	NULL	recognition 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since prenatal counselling is now possible , the recognition of this severe familial under-diagnosed disease is of the upmost importance .
	manualset3
136881	3	407055	5	NULL	NULL	0	NULL	severe familial under-diagnosed disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Since prenatal counselling is now possible , the recognition of this severe familial under-diagnosed disease is of the upmost importance .
	manualset3
136882	1	407056	5	NULL	NULL	0	NULL	progesterone levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since progesterone levels are elevated during these periods we sought to determine how progesterone modulates glycodelin gene expression .
	manualset3
136883	2	407056	5	NULL	NULL	0	NULL	periods 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Since progesterone levels are elevated during these periods we sought to determine how progesterone modulates glycodelin gene expression .
	manualset3
136884	3	407056	5	NULL	NULL	0	NULL	progesterone 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Since progesterone levels are elevated during these periods we sought to determine how progesterone modulates glycodelin gene expression .
	manualset3
136885	4	407056	5	NULL	NULL	0	NULL	glycodelin gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since progesterone levels are elevated during these periods we sought to determine how progesterone modulates glycodelin gene expression .
	manualset3
136886	1	407057	5	NULL	NULL	0	NULL	quinaldine sulfate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Since quinaldine sulfate and tricaine formed type I and II binding spectra , respectively , with brook trout hepatic cytochrome P-450 , these chemicals probably reduced benzo ( a ) pyrene hydroxylase enzyme activity by altering the form ( s ) of cytochrome P-450 responsible for this activity .
	manualset3
136887	2	407057	5	NULL	NULL	0	NULL	tricaine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Since quinaldine sulfate and tricaine formed type I and II binding spectra , respectively , with brook trout hepatic cytochrome P-450 , these chemicals probably reduced benzo ( a ) pyrene hydroxylase enzyme activity by altering the form ( s ) of cytochrome P-450 responsible for this activity .
	manualset3
136888	3	407057	5	NULL	NULL	0	NULL	type I binding spectra	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since quinaldine sulfate and tricaine formed type I and II binding spectra , respectively , with brook trout hepatic cytochrome P-450 , these chemicals probably reduced benzo ( a ) pyrene hydroxylase enzyme activity by altering the form ( s ) of cytochrome P-450 responsible for this activity .
	manualset3
136889	4	407057	5	NULL	NULL	0	NULL	type II binding spectra	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since quinaldine sulfate and tricaine formed type I and II binding spectra , respectively , with brook trout hepatic cytochrome P-450 , these chemicals probably reduced benzo ( a ) pyrene hydroxylase enzyme activity by altering the form ( s ) of cytochrome P-450 responsible for this activity .
	manualset3
136890	5	407057	5	NULL	NULL	0	NULL	brook trout hepatic cytochrome P-450	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since quinaldine sulfate and tricaine formed type I and II binding spectra , respectively , with brook trout hepatic cytochrome P-450 , these chemicals probably reduced benzo ( a ) pyrene hydroxylase enzyme activity by altering the form ( s ) of cytochrome P-450 responsible for this activity .
	manualset3
136891	6	407057	5	NULL	NULL	0	NULL	chemicals 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Since quinaldine sulfate and tricaine formed type I and II binding spectra , respectively , with brook trout hepatic cytochrome P-450 , these chemicals probably reduced benzo ( a ) pyrene hydroxylase enzyme activity by altering the form ( s ) of cytochrome P-450 responsible for this activity .
	manualset3
136892	7	407057	5	NULL	NULL	0	NULL	benzo ( a ) pyrene hydroxylase enzyme activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since quinaldine sulfate and tricaine formed type I and II binding spectra , respectively , with brook trout hepatic cytochrome P-450 , these chemicals probably reduced benzo ( a ) pyrene hydroxylase enzyme activity by altering the form ( s ) of cytochrome P-450 responsible for this activity .
	manualset3
136893	8	407057	5	NULL	NULL	0	NULL	form ( s ) of cytochrome P-450	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since quinaldine sulfate and tricaine formed type I and II binding spectra , respectively , with brook trout hepatic cytochrome P-450 , these chemicals probably reduced benzo ( a ) pyrene hydroxylase enzyme activity by altering the form ( s ) of cytochrome P-450 responsible for this activity .
	manualset3
136894	9	407057	5	NULL	NULL	0	NULL	activity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since quinaldine sulfate and tricaine formed type I and II binding spectra , respectively , with brook trout hepatic cytochrome P-450 , these chemicals probably reduced benzo ( a ) pyrene hydroxylase enzyme activity by altering the form ( s ) of cytochrome P-450 responsible for this activity .
	manualset3
136895	1	407058	5	NULL	NULL	0	NULL	robust immune reactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since robust immune reactions are critical to the survival of humans , the existence of immune variability in the population suggests the existence of competing , alternative phenotypes .
	manualset3
136896	2	407058	5	NULL	NULL	0	NULL	survival 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since robust immune reactions are critical to the survival of humans , the existence of immune variability in the population suggests the existence of competing , alternative phenotypes .
	manualset3
136897	3	407058	5	NULL	NULL	0	NULL	humans 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Since robust immune reactions are critical to the survival of humans , the existence of immune variability in the population suggests the existence of competing , alternative phenotypes .
	manualset3
136898	4	407058	5	NULL	NULL	0	NULL	existence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since robust immune reactions are critical to the survival of humans , the existence of immune variability in the population suggests the existence of competing , alternative phenotypes .
	manualset3
136899	5	407058	5	NULL	NULL	0	NULL	immune variability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since robust immune reactions are critical to the survival of humans , the existence of immune variability in the population suggests the existence of competing , alternative phenotypes .
	manualset3
136900	6	407058	5	NULL	NULL	0	NULL	population 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since robust immune reactions are critical to the survival of humans , the existence of immune variability in the population suggests the existence of competing , alternative phenotypes .
	manualset3
136901	7	407058	5	NULL	NULL	0	NULL	existence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since robust immune reactions are critical to the survival of humans , the existence of immune variability in the population suggests the existence of competing , alternative phenotypes .
	manualset3
136902	8	407058	5	NULL	NULL	0	NULL	competing , alternative phenotypes	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since robust immune reactions are critical to the survival of humans , the existence of immune variability in the population suggests the existence of competing , alternative phenotypes .
	manualset3
136903	1	407059	5	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of characterized polypeptide hormones have been localized in specific gastroenteropancreatic endocrine cells .
	manualset3
136904	2	407059	5	NULL	NULL	0	NULL	characterized polypeptide hormones	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of characterized polypeptide hormones have been localized in specific gastroenteropancreatic endocrine cells .
	manualset3
136905	3	407059	5	NULL	NULL	0	NULL	specific gastroenteropancreatic endocrine cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of characterized polypeptide hormones have been localized in specific gastroenteropancreatic endocrine cells .
	manualset3
136906	1	407060	5	NULL	NULL	0	NULL	cannabinoids 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Since select cannabinoids have anti-inflammatory properties , cross the blood-brain barrier , and target specific receptors , they have potential to serve as agents for dampening untoward neuroimmune responses .
	manualset3
136907	2	407060	5	NULL	NULL	0	NULL	anti-inflammatory properties	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since select cannabinoids have anti-inflammatory properties , cross the blood-brain barrier , and target specific receptors , they have potential to serve as agents for dampening untoward neuroimmune responses .
	manualset3
136908	3	407060	5	NULL	NULL	0	NULL	blood-brain barrier	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Since select cannabinoids have anti-inflammatory properties , cross the blood-brain barrier , and target specific receptors , they have potential to serve as agents for dampening untoward neuroimmune responses .
	manualset3
136909	4	407060	5	NULL	NULL	0	NULL	specific receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since select cannabinoids have anti-inflammatory properties , cross the blood-brain barrier , and target specific receptors , they have potential to serve as agents for dampening untoward neuroimmune responses .
	manualset3
136910	5	407060	5	NULL	NULL	0	NULL	agents 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since select cannabinoids have anti-inflammatory properties , cross the blood-brain barrier , and target specific receptors , they have potential to serve as agents for dampening untoward neuroimmune responses .
	manualset3
136911	6	407060	5	NULL	NULL	0	NULL	neuroimmune responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since select cannabinoids have anti-inflammatory properties , cross the blood-brain barrier , and target specific receptors , they have potential to serve as agents for dampening untoward neuroimmune responses .
	manualset3
136912	1	407061	5	NULL	NULL	0	NULL	separation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since separation of substrate from biological components is required to increase the assay sensitivity and to achieve an accurate assay of beta-lactamase activity , high performance liquid chromatography ( HPLC ) was used for separation and analysis of the substrates ( cephaloridine for cephalosporinase , benzylpenicillin for penicillinase and cefuloxime for cefuloximase ) .
	manualset3
136913	2	407061	5	NULL	NULL	0	NULL	substrate 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since separation of substrate from biological components is required to increase the assay sensitivity and to achieve an accurate assay of beta-lactamase activity , high performance liquid chromatography ( HPLC ) was used for separation and analysis of the substrates ( cephaloridine for cephalosporinase , benzylpenicillin for penicillinase and cefuloxime for cefuloximase ) .
	manualset3
136914	3	407061	5	NULL	NULL	0	NULL	biological components 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since separation of substrate from biological components is required to increase the assay sensitivity and to achieve an accurate assay of beta-lactamase activity , high performance liquid chromatography ( HPLC ) was used for separation and analysis of the substrates ( cephaloridine for cephalosporinase , benzylpenicillin for penicillinase and cefuloxime for cefuloximase ) .
	manualset3
136916	5	407061	5	NULL	NULL	0	NULL	assay sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since separation of substrate from biological components is required to increase the assay sensitivity and to achieve an accurate assay of beta-lactamase activity , high performance liquid chromatography ( HPLC ) was used for separation and analysis of the substrates ( cephaloridine for cephalosporinase , benzylpenicillin for penicillinase and cefuloxime for cefuloximase ) .
	manualset3
136917	6	407061	5	NULL	NULL	0	NULL	accurate assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since separation of substrate from biological components is required to increase the assay sensitivity and to achieve an accurate assay of beta-lactamase activity , high performance liquid chromatography ( HPLC ) was used for separation and analysis of the substrates ( cephaloridine for cephalosporinase , benzylpenicillin for penicillinase and cefuloxime for cefuloximase ) .
	manualset3
136918	7	407061	5	NULL	NULL	0	NULL	beta-lactamase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since separation of substrate from biological components is required to increase the assay sensitivity and to achieve an accurate assay of beta-lactamase activity , high performance liquid chromatography ( HPLC ) was used for separation and analysis of the substrates ( cephaloridine for cephalosporinase , benzylpenicillin for penicillinase and cefuloxime for cefuloximase ) .
	manualset3
136919	8	407061	5	NULL	NULL	0	NULL	high performance liquid chromatography ( HPLC )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since separation of substrate from biological components is required to increase the assay sensitivity and to achieve an accurate assay of beta-lactamase activity , high performance liquid chromatography ( HPLC ) was used for separation and analysis of the substrates ( cephaloridine for cephalosporinase , benzylpenicillin for penicillinase and cefuloxime for cefuloximase ) .
	manualset3
136920	9	407061	5	NULL	NULL	NULL	NULL	separation 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Since separation of substrate from biological components is required to increase the assay sensitivity and to achieve an accurate assay of beta-lactamase activity , high performance liquid chromatography ( HPLC ) was used for separation and analysis of the substrates ( cephaloridine for cephalosporinase , benzylpenicillin for penicillinase and cefuloxime for cefuloximase ) .
	manualset3
136921	10	407061	5	NULL	NULL	0	NULL	analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since separation of substrate from biological components is required to increase the assay sensitivity and to achieve an accurate assay of beta-lactamase activity , high performance liquid chromatography ( HPLC ) was used for separation and analysis of the substrates ( cephaloridine for cephalosporinase , benzylpenicillin for penicillinase and cefuloxime for cefuloximase ) .
	manualset3
136922	11	407061	5	NULL	NULL	0	NULL	substrates 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since separation of substrate from biological components is required to increase the assay sensitivity and to achieve an accurate assay of beta-lactamase activity , high performance liquid chromatography ( HPLC ) was used for separation and analysis of the substrates ( cephaloridine for cephalosporinase , benzylpenicillin for penicillinase and cefuloxime for cefuloximase ) .
	manualset3
136923	12	407061	5	NULL	NULL	0	NULL	cephaloridine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Since separation of substrate from biological components is required to increase the assay sensitivity and to achieve an accurate assay of beta-lactamase activity , high performance liquid chromatography ( HPLC ) was used for separation and analysis of the substrates ( cephaloridine for cephalosporinase , benzylpenicillin for penicillinase and cefuloxime for cefuloximase ) .
	manualset3
136924	13	407061	5	NULL	NULL	0	NULL	cephalosporinase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Since separation of substrate from biological components is required to increase the assay sensitivity and to achieve an accurate assay of beta-lactamase activity , high performance liquid chromatography ( HPLC ) was used for separation and analysis of the substrates ( cephaloridine for cephalosporinase , benzylpenicillin for penicillinase and cefuloxime for cefuloximase ) .
	manualset3
136925	14	407061	5	NULL	NULL	0	NULL	benzylpenicillin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Since separation of substrate from biological components is required to increase the assay sensitivity and to achieve an accurate assay of beta-lactamase activity , high performance liquid chromatography ( HPLC ) was used for separation and analysis of the substrates ( cephaloridine for cephalosporinase , benzylpenicillin for penicillinase and cefuloxime for cefuloximase ) .
	manualset3
136926	15	407061	5	NULL	NULL	0	NULL	penicillinase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Since separation of substrate from biological components is required to increase the assay sensitivity and to achieve an accurate assay of beta-lactamase activity , high performance liquid chromatography ( HPLC ) was used for separation and analysis of the substrates ( cephaloridine for cephalosporinase , benzylpenicillin for penicillinase and cefuloxime for cefuloximase ) .
	manualset3
136927	16	407061	5	NULL	NULL	0	NULL	cefuloxime 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Since separation of substrate from biological components is required to increase the assay sensitivity and to achieve an accurate assay of beta-lactamase activity , high performance liquid chromatography ( HPLC ) was used for separation and analysis of the substrates ( cephaloridine for cephalosporinase , benzylpenicillin for penicillinase and cefuloxime for cefuloximase ) .
	manualset3
136928	17	407061	5	NULL	NULL	0	NULL	cefuloximase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Since separation of substrate from biological components is required to increase the assay sensitivity and to achieve an accurate assay of beta-lactamase activity , high performance liquid chromatography ( HPLC ) was used for separation and analysis of the substrates ( cephaloridine for cephalosporinase , benzylpenicillin for penicillinase and cefuloxime for cefuloximase ) .
	manualset3
136929	1	407062	5	NULL	NULL	0	NULL	somatostatin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Since somatostatin is a local hormone controlling gastric acid secretion and gastrin release , quantitative histopological distribution of the G-cells and D-cells in the canine whole stomach was investigated by the specific immunoperoxidase staining technique .
	manualset3
136930	2	407062	5	NULL	NULL	0	NULL	local hormone	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Since somatostatin is a local hormone controlling gastric acid secretion and gastrin release , quantitative histopological distribution of the G-cells and D-cells in the canine whole stomach was investigated by the specific immunoperoxidase staining technique .
	manualset3
136931	3	407062	5	NULL	NULL	NULL	NULL	gastric acid secretion	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Since somatostatin is a local hormone controlling gastric acid secretion and gastrin release , quantitative histopological distribution of the G-cells and D-cells in the canine whole stomach was investigated by the specific immunoperoxidase staining technique .
	manualset3
136932	4	407062	5	NULL	NULL	0	NULL	gastrin release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since somatostatin is a local hormone controlling gastric acid secretion and gastrin release , quantitative histopological distribution of the G-cells and D-cells in the canine whole stomach was investigated by the specific immunoperoxidase staining technique .
	manualset3
136933	5	407062	5	NULL	NULL	0	NULL	quantitative histopological distribution 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since somatostatin is a local hormone controlling gastric acid secretion and gastrin release , quantitative histopological distribution of the G-cells and D-cells in the canine whole stomach was investigated by the specific immunoperoxidase staining technique .
	manualset3
136934	6	407062	5	NULL	NULL	0	NULL	G-cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Since somatostatin is a local hormone controlling gastric acid secretion and gastrin release , quantitative histopological distribution of the G-cells and D-cells in the canine whole stomach was investigated by the specific immunoperoxidase staining technique .
	manualset3
136935	7	407062	5	NULL	NULL	0	NULL	D-cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Since somatostatin is a local hormone controlling gastric acid secretion and gastrin release , quantitative histopological distribution of the G-cells and D-cells in the canine whole stomach was investigated by the specific immunoperoxidase staining technique .
	manualset3
136936	8	407062	5	NULL	NULL	0	NULL	canine whole stomach	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Since somatostatin is a local hormone controlling gastric acid secretion and gastrin release , quantitative histopological distribution of the G-cells and D-cells in the canine whole stomach was investigated by the specific immunoperoxidase staining technique .
	manualset3
136937	9	407062	5	NULL	NULL	0	NULL	specific immunoperoxidase staining technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since somatostatin is a local hormone controlling gastric acid secretion and gastrin release , quantitative histopological distribution of the G-cells and D-cells in the canine whole stomach was investigated by the specific immunoperoxidase staining technique .
	manualset3
136938	1	407063	5	NULL	NULL	0	NULL	subzero temperatures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since subzero temperatures have no antistyptic effect , additional maneuvers must be performed to control bleeding .
	manualset3
136939	2	407063	5	NULL	NULL	0	NULL	antistyptic effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since subzero temperatures have no antistyptic effect , additional maneuvers must be performed to control bleeding .
	manualset3
136940	3	407063	5	NULL	NULL	0	NULL	maneuvers 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since subzero temperatures have no antistyptic effect , additional maneuvers must be performed to control bleeding .
	manualset3
136941	4	407063	5	NULL	NULL	0	NULL	bleeding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since subzero temperatures have no antistyptic effect , additional maneuvers must be performed to control bleeding .
	manualset3
136942	1	407064	5	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Since that time , the consoles and components of the ECMO circuit have remained fundamentally unchanged ( bladder , rollerpump , silicone membrane oxygenator ) .
	manualset3
136943	2	407064	5	NULL	NULL	0	NULL	consoles 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Since that time , the consoles and components of the ECMO circuit have remained fundamentally unchanged ( bladder , rollerpump , silicone membrane oxygenator ) .
	manualset3
136944	3	407064	5	NULL	NULL	0	NULL	components 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Since that time , the consoles and components of the ECMO circuit have remained fundamentally unchanged ( bladder , rollerpump , silicone membrane oxygenator ) .
	manualset3
136945	4	407064	5	NULL	NULL	0	NULL	ECMO circuit	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Since that time , the consoles and components of the ECMO circuit have remained fundamentally unchanged ( bladder , rollerpump , silicone membrane oxygenator ) .
	manualset3
136946	5	407064	5	NULL	NULL	0	NULL	bladder 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Since that time , the consoles and components of the ECMO circuit have remained fundamentally unchanged ( bladder , rollerpump , silicone membrane oxygenator ) .
	manualset3
136947	6	407064	5	NULL	NULL	0	NULL	rollerpump 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Since that time , the consoles and components of the ECMO circuit have remained fundamentally unchanged ( bladder , rollerpump , silicone membrane oxygenator ) .
	manualset3
136948	7	407064	5	NULL	NULL	0	NULL	silicone membrane oxygenator	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Since that time , the consoles and components of the ECMO circuit have remained fundamentally unchanged ( bladder , rollerpump , silicone membrane oxygenator ) .
	manualset3
136949	1	407065	5	NULL	NULL	0	NULL	NK-1 antagonist	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the NK-1 antagonist produced no systematic changes in responses elicited by the first MO injection , substance P does not seem to be associated directly with the initiation or maintenance of the EMG responses but may be involved if a ` central sensitization ' has been induced by the first MO injection to the TMJ .
	manualset3
136950	2	407065	5	NULL	NULL	0	NULL	systematic changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the NK-1 antagonist produced no systematic changes in responses elicited by the first MO injection , substance P does not seem to be associated directly with the initiation or maintenance of the EMG responses but may be involved if a ` central sensitization ' has been induced by the first MO injection to the TMJ .
	manualset3
136951	3	407065	5	NULL	NULL	0	NULL	responses 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the NK-1 antagonist produced no systematic changes in responses elicited by the first MO injection , substance P does not seem to be associated directly with the initiation or maintenance of the EMG responses but may be involved if a ` central sensitization ' has been induced by the first MO injection to the TMJ .
	manualset3
136952	4	407065	5	NULL	NULL	0	NULL	MO injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the NK-1 antagonist produced no systematic changes in responses elicited by the first MO injection , substance P does not seem to be associated directly with the initiation or maintenance of the EMG responses but may be involved if a ` central sensitization ' has been induced by the first MO injection to the TMJ .
	manualset3
136953	5	407065	5	NULL	NULL	0	NULL	substance P	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the NK-1 antagonist produced no systematic changes in responses elicited by the first MO injection , substance P does not seem to be associated directly with the initiation or maintenance of the EMG responses but may be involved if a ` central sensitization ' has been induced by the first MO injection to the TMJ .
	manualset3
136954	6	407065	5	NULL	NULL	0	NULL	initiation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the NK-1 antagonist produced no systematic changes in responses elicited by the first MO injection , substance P does not seem to be associated directly with the initiation or maintenance of the EMG responses but may be involved if a ` central sensitization ' has been induced by the first MO injection to the TMJ .
	manualset3
136955	7	407065	5	NULL	NULL	0	NULL	maintenance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the NK-1 antagonist produced no systematic changes in responses elicited by the first MO injection , substance P does not seem to be associated directly with the initiation or maintenance of the EMG responses but may be involved if a ` central sensitization ' has been induced by the first MO injection to the TMJ .
	manualset3
136956	8	407065	5	NULL	NULL	0	NULL	EMG responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the NK-1 antagonist produced no systematic changes in responses elicited by the first MO injection , substance P does not seem to be associated directly with the initiation or maintenance of the EMG responses but may be involved if a ` central sensitization ' has been induced by the first MO injection to the TMJ .
	manualset3
136957	9	407065	5	NULL	NULL	0	NULL	central sensitization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the NK-1 antagonist produced no systematic changes in responses elicited by the first MO injection , substance P does not seem to be associated directly with the initiation or maintenance of the EMG responses but may be involved if a ` central sensitization ' has been induced by the first MO injection to the TMJ .
	manualset3
136958	10	407065	5	NULL	NULL	0	NULL	MO injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the NK-1 antagonist produced no systematic changes in responses elicited by the first MO injection , substance P does not seem to be associated directly with the initiation or maintenance of the EMG responses but may be involved if a ` central sensitization ' has been induced by the first MO injection to the TMJ .
	manualset3
136959	11	407065	5	NULL	NULL	0	NULL	TMJ 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the NK-1 antagonist produced no systematic changes in responses elicited by the first MO injection , substance P does not seem to be associated directly with the initiation or maintenance of the EMG responses but may be involved if a ` central sensitization ' has been induced by the first MO injection to the TMJ .
	manualset3
136960	1	407066	5	NULL	NULL	0	NULL	Nuffield report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the Nuffield and DARG reports of the last decade urged consideration of manpower issues within dentistry , the ensuing change from often small , single-handed practice , to larger team approaches has resulted in significant changes in service delivery .
	manualset3
136961	2	407066	5	NULL	NULL	0	NULL	DARG report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the Nuffield and DARG reports of the last decade urged consideration of manpower issues within dentistry , the ensuing change from often small , single-handed practice , to larger team approaches has resulted in significant changes in service delivery .
	manualset3
136962	3	407066	5	NULL	NULL	0	NULL	last decade	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the Nuffield and DARG reports of the last decade urged consideration of manpower issues within dentistry , the ensuing change from often small , single-handed practice , to larger team approaches has resulted in significant changes in service delivery .
	manualset3
136963	4	407066	5	NULL	NULL	0	NULL	consideration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the Nuffield and DARG reports of the last decade urged consideration of manpower issues within dentistry , the ensuing change from often small , single-handed practice , to larger team approaches has resulted in significant changes in service delivery .
	manualset3
136964	5	407066	5	NULL	NULL	0	NULL	manpower issues 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the Nuffield and DARG reports of the last decade urged consideration of manpower issues within dentistry , the ensuing change from often small , single-handed practice , to larger team approaches has resulted in significant changes in service delivery .
	manualset3
136965	6	407066	5	NULL	NULL	0	NULL	dentistry 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the Nuffield and DARG reports of the last decade urged consideration of manpower issues within dentistry , the ensuing change from often small , single-handed practice , to larger team approaches has resulted in significant changes in service delivery .
	manualset3
136966	7	407066	5	NULL	NULL	0	NULL	ensuing change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the Nuffield and DARG reports of the last decade urged consideration of manpower issues within dentistry , the ensuing change from often small , single-handed practice , to larger team approaches has resulted in significant changes in service delivery .
	manualset3
136967	8	407066	5	NULL	NULL	0	NULL	small , single-handed practice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the Nuffield and DARG reports of the last decade urged consideration of manpower issues within dentistry , the ensuing change from often small , single-handed practice , to larger team approaches has resulted in significant changes in service delivery .
	manualset3
136968	9	407066	5	NULL	NULL	0	NULL	larger team approaches 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the Nuffield and DARG reports of the last decade urged consideration of manpower issues within dentistry , the ensuing change from often small , single-handed practice , to larger team approaches has resulted in significant changes in service delivery .
	manualset3
136969	10	407066	5	NULL	NULL	0	NULL	changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the Nuffield and DARG reports of the last decade urged consideration of manpower issues within dentistry , the ensuing change from often small , single-handed practice , to larger team approaches has resulted in significant changes in service delivery .
	manualset3
136970	11	407066	5	NULL	NULL	0	NULL	service delivery	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the Nuffield and DARG reports of the last decade urged consideration of manpower issues within dentistry , the ensuing change from often small , single-handed practice , to larger team approaches has resulted in significant changes in service delivery .
	manualset3
136971	1	407067	5	NULL	NULL	0	NULL	autoimmune pancreatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the autoimmune pancreatitis was introduced in 1995 , it has been recognized as a form of chronic pancreatitis , which is always associated with autoimmune manifestations .
	manualset3
136972	2	407067	5	NULL	NULL	0	NULL	1995 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the autoimmune pancreatitis was introduced in 1995 , it has been recognized as a form of chronic pancreatitis , which is always associated with autoimmune manifestations .
	manualset3
136973	3	407067	5	NULL	NULL	0	NULL	chronic pancreatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the autoimmune pancreatitis was introduced in 1995 , it has been recognized as a form of chronic pancreatitis , which is always associated with autoimmune manifestations .
	manualset3
136974	4	407067	5	NULL	NULL	0	NULL	autoimmune manifestations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the autoimmune pancreatitis was introduced in 1995 , it has been recognized as a form of chronic pancreatitis , which is always associated with autoimmune manifestations .
	manualset3
136975	1	407068	5	NULL	NULL	0	NULL	completion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the completion of the high-quality sequence of its genome , the international community is deploying efforts to identify the function of the 30-40 , 000 nontransposable element genes of rice .
	manualset3
136976	2	407068	5	NULL	NULL	0	NULL	high-quality sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the completion of the high-quality sequence of its genome , the international community is deploying efforts to identify the function of the 30-40 , 000 nontransposable element genes of rice .
	manualset3
136977	3	407068	5	NULL	NULL	0	NULL	genome 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the completion of the high-quality sequence of its genome , the international community is deploying efforts to identify the function of the 30-40 , 000 nontransposable element genes of rice .
	manualset3
136978	4	407068	5	NULL	NULL	0	NULL	international community	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the completion of the high-quality sequence of its genome , the international community is deploying efforts to identify the function of the 30-40 , 000 nontransposable element genes of rice .
	manualset3
136979	5	407068	5	NULL	NULL	0	NULL	efforts 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the completion of the high-quality sequence of its genome , the international community is deploying efforts to identify the function of the 30-40 , 000 nontransposable element genes of rice .
	manualset3
136980	6	407068	5	NULL	NULL	0	NULL	function 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the completion of the high-quality sequence of its genome , the international community is deploying efforts to identify the function of the 30-40 , 000 nontransposable element genes of rice .
	manualset3
136981	7	407068	5	NULL	NULL	0	NULL	30-40 , 000	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the completion of the high-quality sequence of its genome , the international community is deploying efforts to identify the function of the 30-40 , 000 nontransposable element genes of rice .
	manualset3
136982	8	407068	5	NULL	NULL	0	NULL	nontransposable element genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the completion of the high-quality sequence of its genome , the international community is deploying efforts to identify the function of the 30-40 , 000 nontransposable element genes of rice .
	manualset3
136983	9	407068	5	NULL	NULL	0	NULL	rice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the completion of the high-quality sequence of its genome , the international community is deploying efforts to identify the function of the 30-40 , 000 nontransposable element genes of rice .
	manualset3
136984	1	407069	5	NULL	NULL	0	NULL	drug 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the drug has only recently been approved , the German experience is limited .
	manualset3
136985	2	407069	5	NULL	NULL	0	NULL	German experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the drug has only recently been approved , the German experience is limited .
	manualset3
136986	1	407070	5	NULL	NULL	0	NULL	ethnic mix	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the ethnic mix of the US population is changing rapidly and it is estimated that by the year 2020 , over 50 % of US population will include non-Caucasian ethnicity , the identification of the mechanism involved in the excessive development of type 2 diabetes in non-Caucasians becomes important .
	manualset3
136987	2	407070	5	NULL	NULL	0	NULL	US population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the ethnic mix of the US population is changing rapidly and it is estimated that by the year 2020 , over 50 % of US population will include non-Caucasian ethnicity , the identification of the mechanism involved in the excessive development of type 2 diabetes in non-Caucasians becomes important .
	manualset3
136988	3	407070	5	NULL	NULL	0	NULL	year 2020	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the ethnic mix of the US population is changing rapidly and it is estimated that by the year 2020 , over 50 % of US population will include non-Caucasian ethnicity , the identification of the mechanism involved in the excessive development of type 2 diabetes in non-Caucasians becomes important .
	manualset3
136989	4	407070	5	NULL	NULL	0	NULL	50 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the ethnic mix of the US population is changing rapidly and it is estimated that by the year 2020 , over 50 % of US population will include non-Caucasian ethnicity , the identification of the mechanism involved in the excessive development of type 2 diabetes in non-Caucasians becomes important .
	manualset3
136990	5	407070	5	NULL	NULL	0	NULL	US population 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the ethnic mix of the US population is changing rapidly and it is estimated that by the year 2020 , over 50 % of US population will include non-Caucasian ethnicity , the identification of the mechanism involved in the excessive development of type 2 diabetes in non-Caucasians becomes important .
	manualset3
136991	6	407070	5	NULL	NULL	0	NULL	non-Caucasian ethnicity	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the ethnic mix of the US population is changing rapidly and it is estimated that by the year 2020 , over 50 % of US population will include non-Caucasian ethnicity , the identification of the mechanism involved in the excessive development of type 2 diabetes in non-Caucasians becomes important .
	manualset3
136992	7	407070	5	NULL	NULL	0	NULL	identification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the ethnic mix of the US population is changing rapidly and it is estimated that by the year 2020 , over 50 % of US population will include non-Caucasian ethnicity , the identification of the mechanism involved in the excessive development of type 2 diabetes in non-Caucasians becomes important .
	manualset3
136993	8	407070	5	NULL	NULL	0	NULL	mechanism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the ethnic mix of the US population is changing rapidly and it is estimated that by the year 2020 , over 50 % of US population will include non-Caucasian ethnicity , the identification of the mechanism involved in the excessive development of type 2 diabetes in non-Caucasians becomes important .
	manualset3
136994	9	407070	5	NULL	NULL	0	NULL	excessive development	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the ethnic mix of the US population is changing rapidly and it is estimated that by the year 2020 , over 50 % of US population will include non-Caucasian ethnicity , the identification of the mechanism involved in the excessive development of type 2 diabetes in non-Caucasians becomes important .
	manualset3
136995	10	407070	5	NULL	NULL	0	NULL	type 2 diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the ethnic mix of the US population is changing rapidly and it is estimated that by the year 2020 , over 50 % of US population will include non-Caucasian ethnicity , the identification of the mechanism involved in the excessive development of type 2 diabetes in non-Caucasians becomes important .
	manualset3
136996	11	407070	5	NULL	NULL	0	NULL	non-Caucasians 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the ethnic mix of the US population is changing rapidly and it is estimated that by the year 2020 , over 50 % of US population will include non-Caucasian ethnicity , the identification of the mechanism involved in the excessive development of type 2 diabetes in non-Caucasians becomes important .
	manualset3
137125	1	407071	5	NULL	NULL	0	NULL	four 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the four pluronic polyols were composed of identical chemical constituents , we proposed that difference in their activities as adjuvants were due to variation in their physicochemical properties .
	manualset3
137126	2	407071	5	NULL	NULL	0	NULL	pluronic polyols	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the four pluronic polyols were composed of identical chemical constituents , we proposed that difference in their activities as adjuvants were due to variation in their physicochemical properties .
	manualset3
137127	3	407071	5	NULL	NULL	0	NULL	identical chemical constituents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the four pluronic polyols were composed of identical chemical constituents , we proposed that difference in their activities as adjuvants were due to variation in their physicochemical properties .
	manualset3
137131	4	407071	5	NULL	NULL	0	NULL	difference 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the four pluronic polyols were composed of identical chemical constituents , we proposed that difference in their activities as adjuvants were due to variation in their physicochemical properties .
	manualset3
137132	5	407071	5	NULL	NULL	0	NULL	activities 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the four pluronic polyols were composed of identical chemical constituents , we proposed that difference in their activities as adjuvants were due to variation in their physicochemical properties .
	manualset3
137133	6	407071	5	NULL	NULL	0	NULL	adjuvants 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the four pluronic polyols were composed of identical chemical constituents , we proposed that difference in their activities as adjuvants were due to variation in their physicochemical properties .
	manualset3
137134	7	407071	5	NULL	NULL	0	NULL	variation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the four pluronic polyols were composed of identical chemical constituents , we proposed that difference in their activities as adjuvants were due to variation in their physicochemical properties .
	manualset3
137135	8	407071	5	NULL	NULL	0	NULL	physicochemical properties 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the four pluronic polyols were composed of identical chemical constituents , we proposed that difference in their activities as adjuvants were due to variation in their physicochemical properties .
	manualset3
137136	1	407072	5	NULL	NULL	0	NULL	impact 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the impact produces shear stresses larger than the yield stress , the material in the vicinity of the impact becomes fluidized .
	manualset3
137137	2	407072	5	NULL	NULL	0	NULL	shear stresses	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the impact produces shear stresses larger than the yield stress , the material in the vicinity of the impact becomes fluidized .
	manualset3
137138	3	407072	5	NULL	NULL	0	NULL	stress	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the impact produces shear stresses larger than the yield stress , the material in the vicinity of the impact becomes fluidized .
	manualset3
137139	4	407072	5	NULL	NULL	0	NULL	material 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the impact produces shear stresses larger than the yield stress , the material in the vicinity of the impact becomes fluidized .
	manualset3
137153	5	407072	5	NULL	NULL	NULL	NULL	vicinity 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Since the impact produces shear stresses larger than the yield stress , the material in the vicinity of the impact becomes fluidized .
	manualset3
137154	6	407072	5	NULL	NULL	0	NULL	impact 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the impact produces shear stresses larger than the yield stress , the material in the vicinity of the impact becomes fluidized .
	manualset3
137155	1	407073	5	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the increase in protein synthesis is preceded by an increase in RNA synthesis , the two processes might be related .
	manualset3
137156	2	407073	5	NULL	NULL	0	NULL	protein synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the increase in protein synthesis is preceded by an increase in RNA synthesis , the two processes might be related .
	manualset3
137157	3	407073	5	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the increase in protein synthesis is preceded by an increase in RNA synthesis , the two processes might be related .
	manualset3
137158	4	407073	5	NULL	NULL	0	NULL	RNA synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the increase in protein synthesis is preceded by an increase in RNA synthesis , the two processes might be related .
	manualset3
137159	5	407073	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the increase in protein synthesis is preceded by an increase in RNA synthesis , the two processes might be related .
	manualset3
137160	6	407073	5	NULL	NULL	0	NULL	processes 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the increase in protein synthesis is preceded by an increase in RNA synthesis , the two processes might be related .
	manualset3
137161	1	407074	5	NULL	NULL	0	NULL	inhibition 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the inhibition of HDACs leads to growth arrest , differentiation or apoptosis of tumor cell lines , HDACs are promising targets for cancer therapy .
	manualset3
137162	2	407074	5	NULL	NULL	0	NULL	HDACs 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the inhibition of HDACs leads to growth arrest , differentiation or apoptosis of tumor cell lines , HDACs are promising targets for cancer therapy .
	manualset3
137163	3	407074	5	NULL	NULL	0	NULL	growth arrest	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the inhibition of HDACs leads to growth arrest , differentiation or apoptosis of tumor cell lines , HDACs are promising targets for cancer therapy .
	manualset3
137164	4	407074	5	NULL	NULL	0	NULL	differentiation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the inhibition of HDACs leads to growth arrest , differentiation or apoptosis of tumor cell lines , HDACs are promising targets for cancer therapy .
	manualset3
137165	5	407074	5	NULL	NULL	0	NULL	apoptosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the inhibition of HDACs leads to growth arrest , differentiation or apoptosis of tumor cell lines , HDACs are promising targets for cancer therapy .
	manualset3
137166	6	407074	5	NULL	NULL	0	NULL	tumor cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the inhibition of HDACs leads to growth arrest , differentiation or apoptosis of tumor cell lines , HDACs are promising targets for cancer therapy .
	manualset3
137168	7	407074	5	NULL	NULL	0	NULL	HDACs 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the inhibition of HDACs leads to growth arrest , differentiation or apoptosis of tumor cell lines , HDACs are promising targets for cancer therapy .
	manualset3
137169	8	407074	5	NULL	NULL	0	NULL	promising targets	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the inhibition of HDACs leads to growth arrest , differentiation or apoptosis of tumor cell lines , HDACs are promising targets for cancer therapy .
	manualset3
137171	9	407074	5	NULL	NULL	0	NULL	cancer therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the inhibition of HDACs leads to growth arrest , differentiation or apoptosis of tumor cell lines , HDACs are promising targets for cancer therapy .
	manualset3
137176	1	407075	5	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of dietary elements and foods have been reported to be either risk or protective factors for the development of dementia and Alzheimer disease ( AD ) .
	manualset3
137177	2	407075	5	NULL	NULL	0	NULL	dietary elements	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of dietary elements and foods have been reported to be either risk or protective factors for the development of dementia and Alzheimer disease ( AD ) .
	manualset3
137178	3	407075	5	NULL	NULL	0	NULL	foods 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of dietary elements and foods have been reported to be either risk or protective factors for the development of dementia and Alzheimer disease ( AD ) .
	manualset3
137179	4	407075	5	NULL	NULL	NULL	NULL	risk 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A number of dietary elements and foods have been reported to be either risk or protective factors for the development of dementia and Alzheimer disease ( AD ) .
	manualset3
137181	5	407075	5	NULL	NULL	0	NULL	protective factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of dietary elements and foods have been reported to be either risk or protective factors for the development of dementia and Alzheimer disease ( AD ) .
	manualset3
137182	6	407075	5	NULL	NULL	0	NULL	development 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of dietary elements and foods have been reported to be either risk or protective factors for the development of dementia and Alzheimer disease ( AD ) .
	manualset3
137183	7	407075	5	NULL	NULL	0	NULL	dementia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of dietary elements and foods have been reported to be either risk or protective factors for the development of dementia and Alzheimer disease ( AD ) .
	manualset3
137185	8	407075	5	NULL	NULL	0	NULL	Alzheimer disease ( AD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of dietary elements and foods have been reported to be either risk or protective factors for the development of dementia and Alzheimer disease ( AD ) .
	manualset3
137186	1	407076	5	NULL	NULL	NULL	NULL	observation 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Since the observation , by a semiquantitative bioassay , of diminished levels of thymulin in immunodeficiency and autoimmune disease , new data obtained by radioimmunoassay have not only confirmed previous observations but also demonstrated that thymulin plays a role in the interaction between the immune system and the neuro-endocrine system .
	manualset3
137187	2	407076	5	NULL	NULL	0	NULL	semiquantitative bioassay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the observation , by a semiquantitative bioassay , of diminished levels of thymulin in immunodeficiency and autoimmune disease , new data obtained by radioimmunoassay have not only confirmed previous observations but also demonstrated that thymulin plays a role in the interaction between the immune system and the neuro-endocrine system .
	manualset3
137189	3	407076	5	NULL	NULL	0	NULL	diminished levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the observation , by a semiquantitative bioassay , of diminished levels of thymulin in immunodeficiency and autoimmune disease , new data obtained by radioimmunoassay have not only confirmed previous observations but also demonstrated that thymulin plays a role in the interaction between the immune system and the neuro-endocrine system .
	manualset3
137192	4	407076	5	NULL	NULL	0	NULL	thymulin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the observation , by a semiquantitative bioassay , of diminished levels of thymulin in immunodeficiency and autoimmune disease , new data obtained by radioimmunoassay have not only confirmed previous observations but also demonstrated that thymulin plays a role in the interaction between the immune system and the neuro-endocrine system .
	manualset3
137193	5	407076	5	NULL	NULL	0	NULL	immunodeficiency 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the observation , by a semiquantitative bioassay , of diminished levels of thymulin in immunodeficiency and autoimmune disease , new data obtained by radioimmunoassay have not only confirmed previous observations but also demonstrated that thymulin plays a role in the interaction between the immune system and the neuro-endocrine system .
	manualset3
137194	6	407076	5	NULL	NULL	0	NULL	autoimmune disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the observation , by a semiquantitative bioassay , of diminished levels of thymulin in immunodeficiency and autoimmune disease , new data obtained by radioimmunoassay have not only confirmed previous observations but also demonstrated that thymulin plays a role in the interaction between the immune system and the neuro-endocrine system .
	manualset3
137195	7	407076	5	NULL	NULL	0	NULL	new data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the observation , by a semiquantitative bioassay , of diminished levels of thymulin in immunodeficiency and autoimmune disease , new data obtained by radioimmunoassay have not only confirmed previous observations but also demonstrated that thymulin plays a role in the interaction between the immune system and the neuro-endocrine system .
	manualset3
137196	8	407076	5	NULL	NULL	0	NULL	radioimmunoassay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the observation , by a semiquantitative bioassay , of diminished levels of thymulin in immunodeficiency and autoimmune disease , new data obtained by radioimmunoassay have not only confirmed previous observations but also demonstrated that thymulin plays a role in the interaction between the immune system and the neuro-endocrine system .
	manualset3
137197	9	407076	5	NULL	NULL	0	NULL	previous observations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the observation , by a semiquantitative bioassay , of diminished levels of thymulin in immunodeficiency and autoimmune disease , new data obtained by radioimmunoassay have not only confirmed previous observations but also demonstrated that thymulin plays a role in the interaction between the immune system and the neuro-endocrine system .
	manualset3
137198	10	407076	5	NULL	NULL	0	NULL	thymulin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the observation , by a semiquantitative bioassay , of diminished levels of thymulin in immunodeficiency and autoimmune disease , new data obtained by radioimmunoassay have not only confirmed previous observations but also demonstrated that thymulin plays a role in the interaction between the immune system and the neuro-endocrine system .
	manualset3
137199	11	407076	5	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the observation , by a semiquantitative bioassay , of diminished levels of thymulin in immunodeficiency and autoimmune disease , new data obtained by radioimmunoassay have not only confirmed previous observations but also demonstrated that thymulin plays a role in the interaction between the immune system and the neuro-endocrine system .
	manualset3
137200	12	407076	5	NULL	NULL	0	NULL	interaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the observation , by a semiquantitative bioassay , of diminished levels of thymulin in immunodeficiency and autoimmune disease , new data obtained by radioimmunoassay have not only confirmed previous observations but also demonstrated that thymulin plays a role in the interaction between the immune system and the neuro-endocrine system .
	manualset3
137201	13	407076	5	NULL	NULL	0	NULL	immune system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the observation , by a semiquantitative bioassay , of diminished levels of thymulin in immunodeficiency and autoimmune disease , new data obtained by radioimmunoassay have not only confirmed previous observations but also demonstrated that thymulin plays a role in the interaction between the immune system and the neuro-endocrine system .
	manualset3
137202	14	407076	5	NULL	NULL	0	NULL	neuro-endocrine system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the observation , by a semiquantitative bioassay , of diminished levels of thymulin in immunodeficiency and autoimmune disease , new data obtained by radioimmunoassay have not only confirmed previous observations but also demonstrated that thymulin plays a role in the interaction between the immune system and the neuro-endocrine system .
	manualset3
137203	1	407077	5	NULL	NULL	NULL	NULL	predominant fiber type ( FOG )	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Since the predominant fiber type ( FOG ) is adapted for fast contraction and fatigue resistance , the stapedius muscle of the cat is probably capable of fast repetitive contractions , a conclusion that fits well with much of the physiological data .
	manualset3
137204	2	407077	5	NULL	NULL	0	NULL	fast contraction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the predominant fiber type ( FOG ) is adapted for fast contraction and fatigue resistance , the stapedius muscle of the cat is probably capable of fast repetitive contractions , a conclusion that fits well with much of the physiological data .
	manualset3
137205	3	407077	5	NULL	NULL	0	NULL	fatigue resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the predominant fiber type ( FOG ) is adapted for fast contraction and fatigue resistance , the stapedius muscle of the cat is probably capable of fast repetitive contractions , a conclusion that fits well with much of the physiological data .
	manualset3
137206	4	407077	5	NULL	NULL	0	NULL	stapedius muscle	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the predominant fiber type ( FOG ) is adapted for fast contraction and fatigue resistance , the stapedius muscle of the cat is probably capable of fast repetitive contractions , a conclusion that fits well with much of the physiological data .
	manualset3
137207	5	407077	5	NULL	NULL	0	NULL	cat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the predominant fiber type ( FOG ) is adapted for fast contraction and fatigue resistance , the stapedius muscle of the cat is probably capable of fast repetitive contractions , a conclusion that fits well with much of the physiological data .
	manualset3
137208	6	407077	5	NULL	NULL	0	NULL	fast repetitive contractions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the predominant fiber type ( FOG ) is adapted for fast contraction and fatigue resistance , the stapedius muscle of the cat is probably capable of fast repetitive contractions , a conclusion that fits well with much of the physiological data .
	manualset3
137209	7	407077	5	NULL	NULL	0	NULL	conclusion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the predominant fiber type ( FOG ) is adapted for fast contraction and fatigue resistance , the stapedius muscle of the cat is probably capable of fast repetitive contractions , a conclusion that fits well with much of the physiological data .
	manualset3
137210	8	407077	5	NULL	NULL	0	NULL	physiological data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the predominant fiber type ( FOG ) is adapted for fast contraction and fatigue resistance , the stapedius muscle of the cat is probably capable of fast repetitive contractions , a conclusion that fits well with much of the physiological data .
	manualset3
137211	1	407078	5	NULL	NULL	0	NULL	radiometer 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the radiometer was designed to carry out many kinds of measurements in a variety of micro - and macroscopic specimens , and since different methods of microscopy or spectroscopy have to be combined in various ways fro the study of any one specimen , no single master-program could fulfill efficiently all foreseeable requirements .
	manualset3
137212	2	407078	5	NULL	NULL	0	NULL	measurements 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the radiometer was designed to carry out many kinds of measurements in a variety of micro - and macroscopic specimens , and since different methods of microscopy or spectroscopy have to be combined in various ways fro the study of any one specimen , no single master-program could fulfill efficiently all foreseeable requirements .
	manualset3
137213	3	407078	5	NULL	NULL	0	NULL	variety 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the radiometer was designed to carry out many kinds of measurements in a variety of micro - and macroscopic specimens , and since different methods of microscopy or spectroscopy have to be combined in various ways fro the study of any one specimen , no single master-program could fulfill efficiently all foreseeable requirements .
	manualset3
137214	4	407078	5	NULL	NULL	0	NULL	microscopic specimens	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the radiometer was designed to carry out many kinds of measurements in a variety of micro - and macroscopic specimens , and since different methods of microscopy or spectroscopy have to be combined in various ways fro the study of any one specimen , no single master-program could fulfill efficiently all foreseeable requirements .
	manualset3
137215	5	407078	5	NULL	NULL	0	NULL	macroscopic specimens	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the radiometer was designed to carry out many kinds of measurements in a variety of micro - and macroscopic specimens , and since different methods of microscopy or spectroscopy have to be combined in various ways fro the study of any one specimen , no single master-program could fulfill efficiently all foreseeable requirements .
	manualset3
137216	6	407078	5	NULL	NULL	0	NULL	methods of microscopy 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the radiometer was designed to carry out many kinds of measurements in a variety of micro - and macroscopic specimens , and since different methods of microscopy or spectroscopy have to be combined in various ways fro the study of any one specimen , no single master-program could fulfill efficiently all foreseeable requirements .
	manualset3
137217	7	407078	5	NULL	NULL	0	NULL	methods of spectroscopy 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the radiometer was designed to carry out many kinds of measurements in a variety of micro - and macroscopic specimens , and since different methods of microscopy or spectroscopy have to be combined in various ways fro the study of any one specimen , no single master-program could fulfill efficiently all foreseeable requirements .
	manualset3
137218	8	407078	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the radiometer was designed to carry out many kinds of measurements in a variety of micro - and macroscopic specimens , and since different methods of microscopy or spectroscopy have to be combined in various ways fro the study of any one specimen , no single master-program could fulfill efficiently all foreseeable requirements .
	manualset3
137219	9	407078	5	NULL	NULL	0	NULL	one 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the radiometer was designed to carry out many kinds of measurements in a variety of micro - and macroscopic specimens , and since different methods of microscopy or spectroscopy have to be combined in various ways fro the study of any one specimen , no single master-program could fulfill efficiently all foreseeable requirements .
	manualset3
137220	10	407078	5	NULL	NULL	0	NULL	specimen 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the radiometer was designed to carry out many kinds of measurements in a variety of micro - and macroscopic specimens , and since different methods of microscopy or spectroscopy have to be combined in various ways fro the study of any one specimen , no single master-program could fulfill efficiently all foreseeable requirements .
	manualset3
137221	11	407078	5	NULL	NULL	0	NULL	master-program	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the radiometer was designed to carry out many kinds of measurements in a variety of micro - and macroscopic specimens , and since different methods of microscopy or spectroscopy have to be combined in various ways fro the study of any one specimen , no single master-program could fulfill efficiently all foreseeable requirements .
	manualset3
137222	12	407078	5	NULL	NULL	0	NULL	foreseeable requirements	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the radiometer was designed to carry out many kinds of measurements in a variety of micro - and macroscopic specimens , and since different methods of microscopy or spectroscopy have to be combined in various ways fro the study of any one specimen , no single master-program could fulfill efficiently all foreseeable requirements .
	manualset3
137223	1	407079	5	NULL	NULL	0	NULL	response patterns	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the response patterns of cells from different regions of spheroids to HN2 , treated either before disaggregation ( intact spheroid ) or after disaggregation ( isolated spheroid cells ) , are similar and the surviving fraction increases from the surface towards the center of the spheroid , cell cycle distribution is thought to be the only factor involved in the cytotoxicity of HN2 towards cells within the spheroids .
	manualset3
137224	2	407079	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the response patterns of cells from different regions of spheroids to HN2 , treated either before disaggregation ( intact spheroid ) or after disaggregation ( isolated spheroid cells ) , are similar and the surviving fraction increases from the surface towards the center of the spheroid , cell cycle distribution is thought to be the only factor involved in the cytotoxicity of HN2 towards cells within the spheroids .
	manualset3
137225	3	407079	5	NULL	NULL	0	NULL	regions 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the response patterns of cells from different regions of spheroids to HN2 , treated either before disaggregation ( intact spheroid ) or after disaggregation ( isolated spheroid cells ) , are similar and the surviving fraction increases from the surface towards the center of the spheroid , cell cycle distribution is thought to be the only factor involved in the cytotoxicity of HN2 towards cells within the spheroids .
	manualset3
137226	4	407079	5	NULL	NULL	0	NULL	spheroids 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the response patterns of cells from different regions of spheroids to HN2 , treated either before disaggregation ( intact spheroid ) or after disaggregation ( isolated spheroid cells ) , are similar and the surviving fraction increases from the surface towards the center of the spheroid , cell cycle distribution is thought to be the only factor involved in the cytotoxicity of HN2 towards cells within the spheroids .
	manualset3
137227	5	407079	5	NULL	NULL	0	NULL	HN2 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the response patterns of cells from different regions of spheroids to HN2 , treated either before disaggregation ( intact spheroid ) or after disaggregation ( isolated spheroid cells ) , are similar and the surviving fraction increases from the surface towards the center of the spheroid , cell cycle distribution is thought to be the only factor involved in the cytotoxicity of HN2 towards cells within the spheroids .
	manualset3
137228	6	407079	5	NULL	NULL	0	NULL	disaggregation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the response patterns of cells from different regions of spheroids to HN2 , treated either before disaggregation ( intact spheroid ) or after disaggregation ( isolated spheroid cells ) , are similar and the surviving fraction increases from the surface towards the center of the spheroid , cell cycle distribution is thought to be the only factor involved in the cytotoxicity of HN2 towards cells within the spheroids .
	manualset3
137229	7	407079	5	NULL	NULL	0	NULL	spheroid 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the response patterns of cells from different regions of spheroids to HN2 , treated either before disaggregation ( intact spheroid ) or after disaggregation ( isolated spheroid cells ) , are similar and the surviving fraction increases from the surface towards the center of the spheroid , cell cycle distribution is thought to be the only factor involved in the cytotoxicity of HN2 towards cells within the spheroids .
	manualset3
137230	8	407079	5	NULL	NULL	0	NULL	disaggregation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the response patterns of cells from different regions of spheroids to HN2 , treated either before disaggregation ( intact spheroid ) or after disaggregation ( isolated spheroid cells ) , are similar and the surviving fraction increases from the surface towards the center of the spheroid , cell cycle distribution is thought to be the only factor involved in the cytotoxicity of HN2 towards cells within the spheroids .
	manualset3
137231	9	407079	5	NULL	NULL	0	NULL	spheroid cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the response patterns of cells from different regions of spheroids to HN2 , treated either before disaggregation ( intact spheroid ) or after disaggregation ( isolated spheroid cells ) , are similar and the surviving fraction increases from the surface towards the center of the spheroid , cell cycle distribution is thought to be the only factor involved in the cytotoxicity of HN2 towards cells within the spheroids .
	manualset3
137232	10	407079	5	NULL	NULL	0	NULL	surviving fraction	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the response patterns of cells from different regions of spheroids to HN2 , treated either before disaggregation ( intact spheroid ) or after disaggregation ( isolated spheroid cells ) , are similar and the surviving fraction increases from the surface towards the center of the spheroid , cell cycle distribution is thought to be the only factor involved in the cytotoxicity of HN2 towards cells within the spheroids .
	manualset3
137233	11	407079	5	NULL	NULL	0	NULL	surface 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the response patterns of cells from different regions of spheroids to HN2 , treated either before disaggregation ( intact spheroid ) or after disaggregation ( isolated spheroid cells ) , are similar and the surviving fraction increases from the surface towards the center of the spheroid , cell cycle distribution is thought to be the only factor involved in the cytotoxicity of HN2 towards cells within the spheroids .
	manualset3
137234	12	407079	5	NULL	NULL	0	NULL	center 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the response patterns of cells from different regions of spheroids to HN2 , treated either before disaggregation ( intact spheroid ) or after disaggregation ( isolated spheroid cells ) , are similar and the surviving fraction increases from the surface towards the center of the spheroid , cell cycle distribution is thought to be the only factor involved in the cytotoxicity of HN2 towards cells within the spheroids .
	manualset3
137235	13	407079	5	NULL	NULL	0	NULL	spheroid 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the response patterns of cells from different regions of spheroids to HN2 , treated either before disaggregation ( intact spheroid ) or after disaggregation ( isolated spheroid cells ) , are similar and the surviving fraction increases from the surface towards the center of the spheroid , cell cycle distribution is thought to be the only factor involved in the cytotoxicity of HN2 towards cells within the spheroids .
	manualset3
137236	14	407079	5	NULL	NULL	0	NULL	cell cycle distribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the response patterns of cells from different regions of spheroids to HN2 , treated either before disaggregation ( intact spheroid ) or after disaggregation ( isolated spheroid cells ) , are similar and the surviving fraction increases from the surface towards the center of the spheroid , cell cycle distribution is thought to be the only factor involved in the cytotoxicity of HN2 towards cells within the spheroids .
	manualset3
137241	15	407079	5	NULL	NULL	0	NULL	factor 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the response patterns of cells from different regions of spheroids to HN2 , treated either before disaggregation ( intact spheroid ) or after disaggregation ( isolated spheroid cells ) , are similar and the surviving fraction increases from the surface towards the center of the spheroid , cell cycle distribution is thought to be the only factor involved in the cytotoxicity of HN2 towards cells within the spheroids .
	manualset3
137242	16	407079	5	NULL	NULL	0	NULL	cytotoxicity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the response patterns of cells from different regions of spheroids to HN2 , treated either before disaggregation ( intact spheroid ) or after disaggregation ( isolated spheroid cells ) , are similar and the surviving fraction increases from the surface towards the center of the spheroid , cell cycle distribution is thought to be the only factor involved in the cytotoxicity of HN2 towards cells within the spheroids .
	manualset3
137243	17	407079	5	NULL	NULL	0	NULL	HN2 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the response patterns of cells from different regions of spheroids to HN2 , treated either before disaggregation ( intact spheroid ) or after disaggregation ( isolated spheroid cells ) , are similar and the surviving fraction increases from the surface towards the center of the spheroid , cell cycle distribution is thought to be the only factor involved in the cytotoxicity of HN2 towards cells within the spheroids .
	manualset3
137244	18	407079	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the response patterns of cells from different regions of spheroids to HN2 , treated either before disaggregation ( intact spheroid ) or after disaggregation ( isolated spheroid cells ) , are similar and the surviving fraction increases from the surface towards the center of the spheroid , cell cycle distribution is thought to be the only factor involved in the cytotoxicity of HN2 towards cells within the spheroids .
	manualset3
137245	19	407079	5	NULL	NULL	0	NULL	spheroids 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the response patterns of cells from different regions of spheroids to HN2 , treated either before disaggregation ( intact spheroid ) or after disaggregation ( isolated spheroid cells ) , are similar and the surviving fraction increases from the surface towards the center of the spheroid , cell cycle distribution is thought to be the only factor involved in the cytotoxicity of HN2 towards cells within the spheroids .
	manualset3
137246	1	407080	5	NULL	NULL	0	NULL	skull 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the skull is not breached , any inflammation that could affect the process being studied is greatly reduced .
	manualset3
137247	2	407080	5	NULL	NULL	0	NULL	inflammation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the skull is not breached , any inflammation that could affect the process being studied is greatly reduced .
	manualset3
137248	3	407080	5	NULL	NULL	0	NULL	affect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the skull is not breached , any inflammation that could affect the process being studied is greatly reduced .
	manualset3
137249	4	407080	5	NULL	NULL	0	NULL	process 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the skull is not breached , any inflammation that could affect the process being studied is greatly reduced .
	manualset3
137250	1	407081	5	NULL	NULL	0	NULL	beginning 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the very beginning , the purpose of growth promotants has been to enhance production efficiency , reduce the cost of production , and improve profitability .
	manualset3
137251	2	407081	5	NULL	NULL	0	NULL	purpose 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the very beginning , the purpose of growth promotants has been to enhance production efficiency , reduce the cost of production , and improve profitability .
	manualset3
137252	3	407081	5	NULL	NULL	0	NULL	growth promotants	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the very beginning , the purpose of growth promotants has been to enhance production efficiency , reduce the cost of production , and improve profitability .
	manualset3
137254	5	407081	5	NULL	NULL	0	NULL	production efficiency	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the very beginning , the purpose of growth promotants has been to enhance production efficiency , reduce the cost of production , and improve profitability .
	manualset3
137256	7	407081	5	NULL	NULL	0	NULL	cost 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the very beginning , the purpose of growth promotants has been to enhance production efficiency , reduce the cost of production , and improve profitability .
	manualset3
137257	8	407081	5	NULL	NULL	0	NULL	production 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the very beginning , the purpose of growth promotants has been to enhance production efficiency , reduce the cost of production , and improve profitability .
	manualset3
137259	10	407081	5	NULL	NULL	0	NULL	profitability 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the very beginning , the purpose of growth promotants has been to enhance production efficiency , reduce the cost of production , and improve profitability .
	manualset3
137260	1	407082	5	NULL	NULL	0	NULL	prevalence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since then , the prevalence of S. mekongi infection has rapidly decreased in each endemic area .
	manualset3
137261	2	407082	5	NULL	NULL	0	NULL	S. mekongi infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since then , the prevalence of S. mekongi infection has rapidly decreased in each endemic area .
	manualset3
137262	3	407082	5	NULL	NULL	0	NULL	endemic area	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Since then , the prevalence of S. mekongi infection has rapidly decreased in each endemic area .
	manualset3
137263	1	407083	5	NULL	NULL	0	NULL	conclusions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since these conclusions are based on the study of a small number of species , the need for sustained investigations on the molecular biology of pollen developmental transformations is emphasized .
	manualset3
137264	2	407083	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since these conclusions are based on the study of a small number of species , the need for sustained investigations on the molecular biology of pollen developmental transformations is emphasized .
	manualset3
137265	3	407083	5	NULL	NULL	0	NULL	small number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since these conclusions are based on the study of a small number of species , the need for sustained investigations on the molecular biology of pollen developmental transformations is emphasized .
	manualset3
137266	4	407083	5	NULL	NULL	0	NULL	species 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Since these conclusions are based on the study of a small number of species , the need for sustained investigations on the molecular biology of pollen developmental transformations is emphasized .
	manualset3
137267	5	407083	5	NULL	NULL	0	NULL	need 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since these conclusions are based on the study of a small number of species , the need for sustained investigations on the molecular biology of pollen developmental transformations is emphasized .
	manualset3
137268	6	407083	5	NULL	NULL	0	NULL	sustained investigations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since these conclusions are based on the study of a small number of species , the need for sustained investigations on the molecular biology of pollen developmental transformations is emphasized .
	manualset3
137269	7	407083	5	NULL	NULL	0	NULL	molecular biology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since these conclusions are based on the study of a small number of species , the need for sustained investigations on the molecular biology of pollen developmental transformations is emphasized .
	manualset3
137270	8	407083	5	NULL	NULL	0	NULL	pollen developmental transformations 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since these conclusions are based on the study of a small number of species , the need for sustained investigations on the molecular biology of pollen developmental transformations is emphasized .
	manualset3
137271	1	407084	5	NULL	NULL	0	NULL	gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Since this gene is very well conserved among eubacteria , we employed a PCR-based approach using primers based on highly conserved regions of ClpC proteins in order to identify homologous genes in other bifidobacterial species .
	manualset3
137272	2	407084	5	NULL	NULL	0	NULL	eubacteria 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Since this gene is very well conserved among eubacteria , we employed a PCR-based approach using primers based on highly conserved regions of ClpC proteins in order to identify homologous genes in other bifidobacterial species .
	manualset3
137273	3	407084	5	NULL	NULL	0	NULL	PCR-based approach 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since this gene is very well conserved among eubacteria , we employed a PCR-based approach using primers based on highly conserved regions of ClpC proteins in order to identify homologous genes in other bifidobacterial species .
	manualset3
137274	4	407084	5	NULL	NULL	0	NULL	primers 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Since this gene is very well conserved among eubacteria , we employed a PCR-based approach using primers based on highly conserved regions of ClpC proteins in order to identify homologous genes in other bifidobacterial species .
	manualset3
137275	5	407084	5	NULL	NULL	0	NULL	highly conserved regions 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Since this gene is very well conserved among eubacteria , we employed a PCR-based approach using primers based on highly conserved regions of ClpC proteins in order to identify homologous genes in other bifidobacterial species .
	manualset3
137276	6	407084	5	NULL	NULL	0	NULL	ClpC proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since this gene is very well conserved among eubacteria , we employed a PCR-based approach using primers based on highly conserved regions of ClpC proteins in order to identify homologous genes in other bifidobacterial species .
	manualset3
137277	7	407084	5	NULL	NULL	0	NULL	identify 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since this gene is very well conserved among eubacteria , we employed a PCR-based approach using primers based on highly conserved regions of ClpC proteins in order to identify homologous genes in other bifidobacterial species .
	manualset3
137278	8	407084	5	NULL	NULL	0	NULL	homologous genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since this gene is very well conserved among eubacteria , we employed a PCR-based approach using primers based on highly conserved regions of ClpC proteins in order to identify homologous genes in other bifidobacterial species .
	manualset3
137279	9	407084	5	NULL	NULL	0	NULL	bifidobacterial species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Since this gene is very well conserved among eubacteria , we employed a PCR-based approach using primers based on highly conserved regions of ClpC proteins in order to identify homologous genes in other bifidobacterial species .
	manualset3
137280	1	407085	5	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of missed ( interval ) cancers have been diagnosed in children who screened negative both in the Japanese program and in Canadian and English studies , indicating that there is a problem with the sensitivity of screening .
	manualset3
137281	2	407085	5	NULL	NULL	0	NULL	missed ( interval ) cancers 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of missed ( interval ) cancers have been diagnosed in children who screened negative both in the Japanese program and in Canadian and English studies , indicating that there is a problem with the sensitivity of screening .
	manualset3
137282	3	407085	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of missed ( interval ) cancers have been diagnosed in children who screened negative both in the Japanese program and in Canadian and English studies , indicating that there is a problem with the sensitivity of screening .
	manualset3
137285	4	407085	5	NULL	NULL	0	NULL	Japanese program	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of missed ( interval ) cancers have been diagnosed in children who screened negative both in the Japanese program and in Canadian and English studies , indicating that there is a problem with the sensitivity of screening .
	manualset3
137286	5	407085	5	NULL	NULL	0	NULL	Canadian studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of missed ( interval ) cancers have been diagnosed in children who screened negative both in the Japanese program and in Canadian and English studies , indicating that there is a problem with the sensitivity of screening .
	manualset3
137287	6	407085	5	NULL	NULL	0	NULL	English studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of missed ( interval ) cancers have been diagnosed in children who screened negative both in the Japanese program and in Canadian and English studies , indicating that there is a problem with the sensitivity of screening .
	manualset3
137288	7	407085	5	NULL	NULL	0	NULL	problem 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of missed ( interval ) cancers have been diagnosed in children who screened negative both in the Japanese program and in Canadian and English studies , indicating that there is a problem with the sensitivity of screening .
	manualset3
137289	8	407085	5	NULL	NULL	0	NULL	sensitivity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of missed ( interval ) cancers have been diagnosed in children who screened negative both in the Japanese program and in Canadian and English studies , indicating that there is a problem with the sensitivity of screening .
	manualset3
137290	9	407085	5	NULL	NULL	0	NULL	screening 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of missed ( interval ) cancers have been diagnosed in children who screened negative both in the Japanese program and in Canadian and English studies , indicating that there is a problem with the sensitivity of screening .
	manualset3
137291	1	407086	5	NULL	NULL	0	NULL	transport 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since transport is arrested in early endosomes upon inhibition of vesicle acidification , the data also suggest that productive uncoating takes place from early endocytic compartments .
	manualset3
137292	2	407086	5	NULL	NULL	0	NULL	early endosomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Since transport is arrested in early endosomes upon inhibition of vesicle acidification , the data also suggest that productive uncoating takes place from early endocytic compartments .
	manualset3
137297	3	407086	5	NULL	NULL	0	NULL	inhibition 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since transport is arrested in early endosomes upon inhibition of vesicle acidification , the data also suggest that productive uncoating takes place from early endocytic compartments .
	manualset3
137300	4	407086	5	NULL	NULL	0	NULL	vesicle acidification	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since transport is arrested in early endosomes upon inhibition of vesicle acidification , the data also suggest that productive uncoating takes place from early endocytic compartments .
	manualset3
137301	5	407086	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Since transport is arrested in early endosomes upon inhibition of vesicle acidification , the data also suggest that productive uncoating takes place from early endocytic compartments .
	manualset3
137302	6	407086	5	NULL	NULL	0	NULL	early endocytic compartments	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Since transport is arrested in early endosomes upon inhibition of vesicle acidification , the data also suggest that productive uncoating takes place from early endocytic compartments .
	manualset3
137305	1	407087	5	NULL	NULL	0	NULL	viable bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Since viable bacteria can persist in tooth cavities regardless of the technique used for caries removal , the objective of the present randomized clinical trial was to examine the microflora of primary teeth treated by complete or partial removal of carious dentin .
	manualset3
137308	2	407087	5	NULL	NULL	0	NULL	 tooth cavities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since viable bacteria can persist in tooth cavities regardless of the technique used for caries removal , the objective of the present randomized clinical trial was to examine the microflora of primary teeth treated by complete or partial removal of carious dentin .
	manualset3
137309	3	407087	5	NULL	NULL	0	NULL	technique 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Since viable bacteria can persist in tooth cavities regardless of the technique used for caries removal , the objective of the present randomized clinical trial was to examine the microflora of primary teeth treated by complete or partial removal of carious dentin .
	manualset3
137332	4	407087	5	NULL	NULL	0	NULL	caries removal	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Since viable bacteria can persist in tooth cavities regardless of the technique used for caries removal , the objective of the present randomized clinical trial was to examine the microflora of primary teeth treated by complete or partial removal of carious dentin .
	manualset3
137334	5	407087	5	NULL	NULL	0	NULL	objective 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since viable bacteria can persist in tooth cavities regardless of the technique used for caries removal , the objective of the present randomized clinical trial was to examine the microflora of primary teeth treated by complete or partial removal of carious dentin .
	manualset3
137335	6	407087	5	NULL	NULL	0	NULL	present randomized clinical trial 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since viable bacteria can persist in tooth cavities regardless of the technique used for caries removal , the objective of the present randomized clinical trial was to examine the microflora of primary teeth treated by complete or partial removal of carious dentin .
	manualset3
137338	8	407087	5	NULL	NULL	0	NULL	microflora 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Since viable bacteria can persist in tooth cavities regardless of the technique used for caries removal , the objective of the present randomized clinical trial was to examine the microflora of primary teeth treated by complete or partial removal of carious dentin .
	manualset3
137340	9	407087	5	NULL	NULL	0	NULL	primary teeth	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Since viable bacteria can persist in tooth cavities regardless of the technique used for caries removal , the objective of the present randomized clinical trial was to examine the microflora of primary teeth treated by complete or partial removal of carious dentin .
	manualset3
137343	10	407087	5	NULL	NULL	0	NULL	complete removal 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Since viable bacteria can persist in tooth cavities regardless of the technique used for caries removal , the objective of the present randomized clinical trial was to examine the microflora of primary teeth treated by complete or partial removal of carious dentin .
	manualset3
137344	11	407087	5	NULL	NULL	0	NULL	partial removal	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Since viable bacteria can persist in tooth cavities regardless of the technique used for caries removal , the objective of the present randomized clinical trial was to examine the microflora of primary teeth treated by complete or partial removal of carious dentin .
	manualset3
137349	12	407087	5	NULL	NULL	0	NULL	carious dentin	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since viable bacteria can persist in tooth cavities regardless of the technique used for caries removal , the objective of the present randomized clinical trial was to examine the microflora of primary teeth treated by complete or partial removal of carious dentin .
	manualset3
137352	1	407088	5	NULL	NULL	0	NULL	wogonin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Since wogonin inhibited dexamethasone-induced DNA fragmentation in a noncompetitive manner , a target of this flavone is unlikely to be an antagonist of glucocorticoid receptor .
	manualset3
137354	2	407088	5	NULL	NULL	0	NULL	dexamethasone-induced DNA fragmentation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since wogonin inhibited dexamethasone-induced DNA fragmentation in a noncompetitive manner , a target of this flavone is unlikely to be an antagonist of glucocorticoid receptor .
	manualset3
137356	3	407088	5	NULL	NULL	0	NULL	noncompetitive manner	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since wogonin inhibited dexamethasone-induced DNA fragmentation in a noncompetitive manner , a target of this flavone is unlikely to be an antagonist of glucocorticoid receptor .
	manualset3
137357	4	407088	5	NULL	NULL	0	NULL	target 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since wogonin inhibited dexamethasone-induced DNA fragmentation in a noncompetitive manner , a target of this flavone is unlikely to be an antagonist of glucocorticoid receptor .
	manualset3
137359	5	407088	5	NULL	NULL	0	NULL	flavone 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Since wogonin inhibited dexamethasone-induced DNA fragmentation in a noncompetitive manner , a target of this flavone is unlikely to be an antagonist of glucocorticoid receptor .
	manualset3
137360	6	407088	5	NULL	NULL	0	NULL	antagonist 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since wogonin inhibited dexamethasone-induced DNA fragmentation in a noncompetitive manner , a target of this flavone is unlikely to be an antagonist of glucocorticoid receptor .
	manualset3
137361	7	407088	5	NULL	NULL	0	NULL	glucocorticoid receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Since wogonin inhibited dexamethasone-induced DNA fragmentation in a noncompetitive manner , a target of this flavone is unlikely to be an antagonist of glucocorticoid receptor .
	manualset3
137392	1	407089	5	NULL	NULL	0	NULL	risk 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since there is less risk of recession and more potential for gain in papillary height , the papillary retention procedure , when possible , may be the procedure of choice in anterior regions .
	manualset3
137393	2	407089	5	NULL	NULL	0	NULL	recession 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since there is less risk of recession and more potential for gain in papillary height , the papillary retention procedure , when possible , may be the procedure of choice in anterior regions .
	manualset3
137394	3	407089	5	NULL	NULL	0	NULL	potential 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since there is less risk of recession and more potential for gain in papillary height , the papillary retention procedure , when possible , may be the procedure of choice in anterior regions .
	manualset3
137395	4	407089	5	NULL	NULL	0	NULL	papillary height	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since there is less risk of recession and more potential for gain in papillary height , the papillary retention procedure , when possible , may be the procedure of choice in anterior regions .
	manualset3
137396	5	407089	5	NULL	NULL	0	NULL	papillary retention procedure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since there is less risk of recession and more potential for gain in papillary height , the papillary retention procedure , when possible , may be the procedure of choice in anterior regions .
	manualset3
137397	6	407089	5	NULL	NULL	0	NULL	procedure 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since there is less risk of recession and more potential for gain in papillary height , the papillary retention procedure , when possible , may be the procedure of choice in anterior regions .
	manualset3
137398	7	407089	5	NULL	NULL	0	NULL	choice 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since there is less risk of recession and more potential for gain in papillary height , the papillary retention procedure , when possible , may be the procedure of choice in anterior regions .
	manualset3
137399	8	407089	5	NULL	NULL	0	NULL	anterior regions	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since there is less risk of recession and more potential for gain in papillary height , the papillary retention procedure , when possible , may be the procedure of choice in anterior regions .
	manualset3
137400	1	407090	5	NULL	NULL	0	NULL	Single-celled parasites 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-celled parasites like Entamoeba , Trypanosoma , Phytophthora and Plasmodium wreak untold havoc on human habitat and health .
	manualset3
137401	2	407090	5	NULL	NULL	0	NULL	Entamoeba 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-celled parasites like Entamoeba , Trypanosoma , Phytophthora and Plasmodium wreak untold havoc on human habitat and health .
	manualset3
137402	3	407090	5	NULL	NULL	0	NULL	Trypanosoma 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-celled parasites like Entamoeba , Trypanosoma , Phytophthora and Plasmodium wreak untold havoc on human habitat and health .
	manualset3
137403	4	407090	5	NULL	NULL	0	NULL	Phytophthora 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-celled parasites like Entamoeba , Trypanosoma , Phytophthora and Plasmodium wreak untold havoc on human habitat and health .
	manualset3
137404	5	407090	5	NULL	NULL	0	NULL	Plasmodium 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-celled parasites like Entamoeba , Trypanosoma , Phytophthora and Plasmodium wreak untold havoc on human habitat and health .
	manualset3
137410	6	407090	5	NULL	NULL	0	NULL	havoc 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-celled parasites like Entamoeba , Trypanosoma , Phytophthora and Plasmodium wreak untold havoc on human habitat and health .
	manualset3
137412	7	407090	5	NULL	NULL	0	NULL	human habitat	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-celled parasites like Entamoeba , Trypanosoma , Phytophthora and Plasmodium wreak untold havoc on human habitat and health .
	manualset3
137413	8	407090	5	NULL	NULL	0	NULL	health 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-celled parasites like Entamoeba , Trypanosoma , Phytophthora and Plasmodium wreak untold havoc on human habitat and health .
	manualset3
137414	1	407091	5	NULL	NULL	NULL	NULL	Single-channel recordings 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Single-channel recordings suggest that the partial efficacy of physostigmine may reflect the low frequency of opening of physostigmine-induced single currents relative to that of ACh-single currents .
	manualset3
137415	2	407091	5	NULL	NULL	0	NULL	partial efficacy	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-channel recordings suggest that the partial efficacy of physostigmine may reflect the low frequency of opening of physostigmine-induced single currents relative to that of ACh-single currents .
	manualset3
137416	3	407091	5	NULL	NULL	0	NULL	physostigmine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-channel recordings suggest that the partial efficacy of physostigmine may reflect the low frequency of opening of physostigmine-induced single currents relative to that of ACh-single currents .
	manualset3
137417	4	407091	5	NULL	NULL	0	NULL	low frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-channel recordings suggest that the partial efficacy of physostigmine may reflect the low frequency of opening of physostigmine-induced single currents relative to that of ACh-single currents .
	manualset3
137418	5	407091	5	NULL	NULL	0	NULL	opening 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-channel recordings suggest that the partial efficacy of physostigmine may reflect the low frequency of opening of physostigmine-induced single currents relative to that of ACh-single currents .
	manualset3
137419	6	407091	5	NULL	NULL	0	NULL	physostigmine-induced single currents 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-channel recordings suggest that the partial efficacy of physostigmine may reflect the low frequency of opening of physostigmine-induced single currents relative to that of ACh-single currents .
	manualset3
137420	7	407091	5	NULL	NULL	0	NULL	ACh-single currents	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-channel recordings suggest that the partial efficacy of physostigmine may reflect the low frequency of opening of physostigmine-induced single currents relative to that of ACh-single currents .
	manualset3
137422	1	407092	5	NULL	NULL	0	NULL	Single-dose pharmacokinetics 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-dose pharmacokinetics of labetalol in healthy young men .
	manualset3
137425	2	407092	5	NULL	NULL	0	NULL	labetalol 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-dose pharmacokinetics of labetalol in healthy young men .
	manualset3
137427	3	407092	5	NULL	NULL	0	NULL	healthy young men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-dose pharmacokinetics of labetalol in healthy young men .
	manualset3
137430	1	407093	5	NULL	NULL	0	NULL	Single-photon emission computed tomography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-photon emission computed tomography with 99mTC-hexamethylpropyleneamineoxide in cirrhotic patients before and after liver transplantation .
	manualset3
137435	2	407093	5	NULL	NULL	0	NULL	99mTC-hexamethylpropyleneamineoxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-photon emission computed tomography with 99mTC-hexamethylpropyleneamineoxide in cirrhotic patients before and after liver transplantation .
	manualset3
137437	3	407093	5	NULL	NULL	0	NULL	cirrhotic patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-photon emission computed tomography with 99mTC-hexamethylpropyleneamineoxide in cirrhotic patients before and after liver transplantation .
	manualset3
137438	4	407093	5	NULL	NULL	0	NULL	liver transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-photon emission computed tomography with 99mTC-hexamethylpropyleneamineoxide in cirrhotic patients before and after liver transplantation .
	manualset3
137440	1	407094	5	NULL	NULL	0	NULL	Single-wavelength anomalous scattering ( SAS ) phasing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-wavelength anomalous scattering ( SAS ) phasing with chromium X-ray radiation opens a new possibility for phasing a protein with data collected in-house and has led to several successful examples of de novo structure solution using only weak anomalous scatterers such as sulfur .
	manualset3
137441	2	407094	5	NULL	NULL	0	NULL	chromium X-ray radiation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-wavelength anomalous scattering ( SAS ) phasing with chromium X-ray radiation opens a new possibility for phasing a protein with data collected in-house and has led to several successful examples of de novo structure solution using only weak anomalous scatterers such as sulfur .
	manualset3
137442	3	407094	5	NULL	NULL	0	NULL	possibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-wavelength anomalous scattering ( SAS ) phasing with chromium X-ray radiation opens a new possibility for phasing a protein with data collected in-house and has led to several successful examples of de novo structure solution using only weak anomalous scatterers such as sulfur .
	manualset3
137443	4	407094	5	NULL	NULL	0	NULL	phasing 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-wavelength anomalous scattering ( SAS ) phasing with chromium X-ray radiation opens a new possibility for phasing a protein with data collected in-house and has led to several successful examples of de novo structure solution using only weak anomalous scatterers such as sulfur .
	manualset3
137444	5	407094	5	NULL	NULL	0	NULL	protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-wavelength anomalous scattering ( SAS ) phasing with chromium X-ray radiation opens a new possibility for phasing a protein with data collected in-house and has led to several successful examples of de novo structure solution using only weak anomalous scatterers such as sulfur .
	manualset3
137445	6	407094	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-wavelength anomalous scattering ( SAS ) phasing with chromium X-ray radiation opens a new possibility for phasing a protein with data collected in-house and has led to several successful examples of de novo structure solution using only weak anomalous scatterers such as sulfur .
	manualset3
137446	7	407094	5	NULL	NULL	0	NULL	in-house	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-wavelength anomalous scattering ( SAS ) phasing with chromium X-ray radiation opens a new possibility for phasing a protein with data collected in-house and has led to several successful examples of de novo structure solution using only weak anomalous scatterers such as sulfur .
	manualset3
137447	8	407094	5	NULL	NULL	0	NULL	successful examples	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-wavelength anomalous scattering ( SAS ) phasing with chromium X-ray radiation opens a new possibility for phasing a protein with data collected in-house and has led to several successful examples of de novo structure solution using only weak anomalous scatterers such as sulfur .
	manualset3
137448	9	407094	5	NULL	NULL	0	NULL	de novo structure solution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-wavelength anomalous scattering ( SAS ) phasing with chromium X-ray radiation opens a new possibility for phasing a protein with data collected in-house and has led to several successful examples of de novo structure solution using only weak anomalous scatterers such as sulfur .
	manualset3
137449	10	407094	5	NULL	NULL	0	NULL	weak anomalous scatterers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-wavelength anomalous scattering ( SAS ) phasing with chromium X-ray radiation opens a new possibility for phasing a protein with data collected in-house and has led to several successful examples of de novo structure solution using only weak anomalous scatterers such as sulfur .
	manualset3
137450	11	407094	5	NULL	NULL	0	NULL	sulfur 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-wavelength anomalous scattering ( SAS ) phasing with chromium X-ray radiation opens a new possibility for phasing a protein with data collected in-house and has led to several successful examples of de novo structure solution using only weak anomalous scatterers such as sulfur .
	manualset3
137451	1	407095	5	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of obstacles to the provision of the SLT service to aphasic people were identified .
	manualset3
137452	2	407095	5	NULL	NULL	0	NULL	obstacles 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of obstacles to the provision of the SLT service to aphasic people were identified .
	manualset3
137453	3	407095	5	NULL	NULL	0	NULL	provision 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of obstacles to the provision of the SLT service to aphasic people were identified .
	manualset3
137454	4	407095	5	NULL	NULL	0	NULL	SLT service	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of obstacles to the provision of the SLT service to aphasic people were identified .
	manualset3
137455	5	407095	5	NULL	NULL	0	NULL	aphasic people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of obstacles to the provision of the SLT service to aphasic people were identified .
	manualset3
137456	1	407096	5	NULL	NULL	0	NULL	Single access surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Single access surgery has the same goal by reducing the number and the size of access incisions .
	manualset3
137457	2	407096	5	NULL	NULL	0	NULL	same goal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Single access surgery has the same goal by reducing the number and the size of access incisions .
	manualset3
137458	3	407096	5	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Single access surgery has the same goal by reducing the number and the size of access incisions .
	manualset3
137459	4	407096	5	NULL	NULL	0	NULL	size 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Single access surgery has the same goal by reducing the number and the size of access incisions .
	manualset3
137460	5	407096	5	NULL	NULL	0	NULL	access incisions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Single access surgery has the same goal by reducing the number and the size of access incisions .
	manualset3
137463	1	407097	5	NULL	NULL	0	NULL	Single and aggregated platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Single and aggregated platelets were adherent to the dialysis membranes , to leukocytes , and to amorphous debris .
	manualset3
137465	2	407097	5	NULL	NULL	0	NULL	dialysis membranes 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Single and aggregated platelets were adherent to the dialysis membranes , to leukocytes , and to amorphous debris .
	manualset3
137466	3	407097	5	NULL	NULL	0	NULL	leukocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Single and aggregated platelets were adherent to the dialysis membranes , to leukocytes , and to amorphous debris .
	manualset3
137467	4	407097	5	NULL	NULL	0	NULL	amorphous debris	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Single and aggregated platelets were adherent to the dialysis membranes , to leukocytes , and to amorphous debris .
	manualset3
137468	1	407098	5	NULL	NULL	0	NULL	Single atrial myocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Single atrial myocytes were enzymatically isolated from the bull-frog as previously described ( Hume & Giles , 1981 ) , and patch-clamp techniques were used in an attempt to identify and separate two inwardly rectifying K + channels in this tissue .
	manualset3
137469	2	407098	5	NULL	NULL	0	NULL	bull-frog	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Single atrial myocytes were enzymatically isolated from the bull-frog as previously described ( Hume & Giles , 1981 ) , and patch-clamp techniques were used in an attempt to identify and separate two inwardly rectifying K + channels in this tissue .
	manualset3
137470	3	407098	5	NULL	NULL	0	NULL	Hume & Giles , 1981	Citation												NULL		0	NULL	NULL	NULL	NULL	NULL	Single atrial myocytes were enzymatically isolated from the bull-frog as previously described ( Hume & Giles , 1981 ) , and patch-clamp techniques were used in an attempt to identify and separate two inwardly rectifying K + channels in this tissue .
	manualset3
137471	4	407098	5	NULL	NULL	0	NULL	patch-clamp techniques 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Single atrial myocytes were enzymatically isolated from the bull-frog as previously described ( Hume & Giles , 1981 ) , and patch-clamp techniques were used in an attempt to identify and separate two inwardly rectifying K + channels in this tissue .
	manualset3
137474	7	407098	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Single atrial myocytes were enzymatically isolated from the bull-frog as previously described ( Hume & Giles , 1981 ) , and patch-clamp techniques were used in an attempt to identify and separate two inwardly rectifying K + channels in this tissue .
	manualset3
137475	8	407098	5	NULL	NULL	0	NULL	inwardly rectifying K + channels 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Single atrial myocytes were enzymatically isolated from the bull-frog as previously described ( Hume & Giles , 1981 ) , and patch-clamp techniques were used in an attempt to identify and separate two inwardly rectifying K + channels in this tissue .
	manualset3
137476	9	407098	5	NULL	NULL	0	NULL	tissue 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Single atrial myocytes were enzymatically isolated from the bull-frog as previously described ( Hume & Giles , 1981 ) , and patch-clamp techniques were used in an attempt to identify and separate two inwardly rectifying K + channels in this tissue .
	manualset3
137477	1	407099	5	NULL	NULL	0	NULL	Single capsulated cyst	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Single capsulated cyst full of pus was surgically removed by using cardio-pulmonary bypass .
	manualset3
137478	2	407099	5	NULL	NULL	0	NULL	pus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Single capsulated cyst full of pus was surgically removed by using cardio-pulmonary bypass .
	manualset3
137480	3	407099	5	NULL	NULL	0	NULL	cardio-pulmonary bypass	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Single capsulated cyst full of pus was surgically removed by using cardio-pulmonary bypass .
	manualset3
137482	1	407100	5	NULL	NULL	0	NULL	Single channel conductance 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Single channel conductance measured in 20 mm external Ca2 + was 5.9 pS .
	manualset3
137485	2	407100	5	NULL	NULL	0	NULL	20 mm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Single channel conductance measured in 20 mm external Ca2 + was 5.9 pS .
	manualset3
137486	3	407100	5	NULL	NULL	0	NULL	 Ca2 + 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Single channel conductance measured in 20 mm external Ca2 + was 5.9 pS .
	manualset3
137487	4	407100	5	NULL	NULL	0	NULL	5.9 pS	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Single channel conductance measured in 20 mm external Ca2 + was 5.9 pS .
	manualset3
137489	1	407101	5	NULL	NULL	0	NULL	Single core polypeptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Single core polypeptide in the reaction center of the photosynthetic bacterium Heliobacillus mobilis : structural implications and relations to other photosystems .
	manualset3
137492	2	407101	5	NULL	NULL	0	NULL	reaction center 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Single core polypeptide in the reaction center of the photosynthetic bacterium Heliobacillus mobilis : structural implications and relations to other photosystems .
	manualset3
137494	3	407101	5	NULL	NULL	0	NULL	photosynthetic bacterium Heliobacillus mobilis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Single core polypeptide in the reaction center of the photosynthetic bacterium Heliobacillus mobilis : structural implications and relations to other photosystems .
	manualset3
137495	4	407101	5	NULL	NULL	0	NULL	structural implications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Single core polypeptide in the reaction center of the photosynthetic bacterium Heliobacillus mobilis : structural implications and relations to other photosystems .
	manualset3
137496	5	407101	5	NULL	NULL	0	NULL	relations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Single core polypeptide in the reaction center of the photosynthetic bacterium Heliobacillus mobilis : structural implications and relations to other photosystems .
	manualset3
137497	6	407101	5	NULL	NULL	0	NULL	photosystems 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Single core polypeptide in the reaction center of the photosynthetic bacterium Heliobacillus mobilis : structural implications and relations to other photosystems .
	manualset3
137501	1	407102	5	NULL	NULL	NULL	NULL	Single donor apheresis 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Single donor apheresis was found to be the major source of platelets in hematology ( 80.8 % , n = 147 ) and oncology ( 86.5 % , n = 45 ) clinics .
	manualset3
137504	2	407102	5	NULL	NULL	0	NULL	major source	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Single donor apheresis was found to be the major source of platelets in hematology ( 80.8 % , n = 147 ) and oncology ( 86.5 % , n = 45 ) clinics .
	manualset3
137505	3	407102	5	NULL	NULL	0	NULL	platelets 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Single donor apheresis was found to be the major source of platelets in hematology ( 80.8 % , n = 147 ) and oncology ( 86.5 % , n = 45 ) clinics .
	manualset3
137506	4	407102	5	NULL	NULL	NULL	NULL	hematology clinics	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Single donor apheresis was found to be the major source of platelets in hematology ( 80.8 % , n = 147 ) and oncology ( 86.5 % , n = 45 ) clinics .
	manualset3
137507	5	407102	5	NULL	NULL	0	NULL	80.8 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Single donor apheresis was found to be the major source of platelets in hematology ( 80.8 % , n = 147 ) and oncology ( 86.5 % , n = 45 ) clinics .
	manualset3
137509	6	407102	5	NULL	NULL	0	NULL	n = 147	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Single donor apheresis was found to be the major source of platelets in hematology ( 80.8 % , n = 147 ) and oncology ( 86.5 % , n = 45 ) clinics .
	manualset3
137512	7	407102	5	NULL	NULL	NULL	NULL	oncology clinics	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Single donor apheresis was found to be the major source of platelets in hematology ( 80.8 % , n = 147 ) and oncology ( 86.5 % , n = 45 ) clinics .
	manualset3
137513	8	407102	5	NULL	NULL	0	NULL	86.5 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Single donor apheresis was found to be the major source of platelets in hematology ( 80.8 % , n = 147 ) and oncology ( 86.5 % , n = 45 ) clinics .
	manualset3
137514	9	407102	5	NULL	NULL	0	NULL	n = 45	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Single donor apheresis was found to be the major source of platelets in hematology ( 80.8 % , n = 147 ) and oncology ( 86.5 % , n = 45 ) clinics .
	manualset3
137517	1	407103	5	NULL	NULL	0	NULL	Single filaments	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Single filaments can stretch to more than 3 times their initial length before breaking , and gels of IF withstand strains greater than 100 % without damage .
	manualset3
137519	3	407103	5	NULL	NULL	0	NULL	 more than 3 times 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Single filaments can stretch to more than 3 times their initial length before breaking , and gels of IF withstand strains greater than 100 % without damage .
	manualset3
137520	4	407103	5	NULL	NULL	0	NULL	initial length 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Single filaments can stretch to more than 3 times their initial length before breaking , and gels of IF withstand strains greater than 100 % without damage .
	manualset3
137521	5	407103	5	NULL	NULL	0	NULL	gels 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Single filaments can stretch to more than 3 times their initial length before breaking , and gels of IF withstand strains greater than 100 % without damage .
	manualset3
137522	6	407103	5	NULL	NULL	0	NULL	IF 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Single filaments can stretch to more than 3 times their initial length before breaking , and gels of IF withstand strains greater than 100 % without damage .
	manualset3
137523	7	407103	5	NULL	NULL	0	NULL	strains 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Single filaments can stretch to more than 3 times their initial length before breaking , and gels of IF withstand strains greater than 100 % without damage .
	manualset3
137524	8	407103	5	NULL	NULL	0	NULL	100 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Single filaments can stretch to more than 3 times their initial length before breaking , and gels of IF withstand strains greater than 100 % without damage .
	manualset3
137525	9	407103	5	NULL	NULL	0	NULL	damage 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Single filaments can stretch to more than 3 times their initial length before breaking , and gels of IF withstand strains greater than 100 % without damage .
	manualset3
137526	1	407104	5	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of other factors , most probably influencing or modifying the use of tobacco and alcohol , were found to be significant also .
	manualset3
137527	2	407104	5	NULL	NULL	0	NULL	factors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of other factors , most probably influencing or modifying the use of tobacco and alcohol , were found to be significant also .
	manualset3
137529	3	407104	5	NULL	NULL	0	NULL	use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of other factors , most probably influencing or modifying the use of tobacco and alcohol , were found to be significant also .
	manualset3
137531	4	407104	5	NULL	NULL	0	NULL	tobacco 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of other factors , most probably influencing or modifying the use of tobacco and alcohol , were found to be significant also .
	manualset3
137533	5	407104	5	NULL	NULL	0	NULL	alcohol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of other factors , most probably influencing or modifying the use of tobacco and alcohol , were found to be significant also .
	manualset3
137534	1	407105	5	NULL	NULL	0	NULL	Single neurons 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Single neurons in the NST were recorded extracellularly and drugs ( 21 nl ) were microinjected into the vicinity of the cell via a multibarrel pipette .
	manualset3
137539	2	407105	5	NULL	NULL	0	NULL	NST 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Single neurons in the NST were recorded extracellularly and drugs ( 21 nl ) were microinjected into the vicinity of the cell via a multibarrel pipette .
	manualset3
137540	3	407105	5	NULL	NULL	0	NULL	drugs ( 21 nl )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Single neurons in the NST were recorded extracellularly and drugs ( 21 nl ) were microinjected into the vicinity of the cell via a multibarrel pipette .
	manualset3
137542	4	407105	5	NULL	NULL	0	NULL	vicinity 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Single neurons in the NST were recorded extracellularly and drugs ( 21 nl ) were microinjected into the vicinity of the cell via a multibarrel pipette .
	manualset3
137544	5	407105	5	NULL	NULL	0	NULL	cell 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Single neurons in the NST were recorded extracellularly and drugs ( 21 nl ) were microinjected into the vicinity of the cell via a multibarrel pipette .
	manualset3
137547	6	407105	5	NULL	NULL	NULL	NULL	multibarrel pipette	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Single neurons in the NST were recorded extracellularly and drugs ( 21 nl ) were microinjected into the vicinity of the cell via a multibarrel pipette .
	manualset3
137548	1	407106	5	NULL	NULL	0	NULL	Single nucleotide polymorphisms ( SNPs )	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Single nucleotide polymorphisms ( SNPs ) in transcription factor binding sites ( TFBSs ) may affect the binding of transcription factors , lead to differences in gene expression and phenotypes and therefore affect susceptibility to environmental exposure .
	manualset3
137549	2	407106	5	NULL	NULL	0	NULL	transcription factor binding sites ( TFBSs ) 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Single nucleotide polymorphisms ( SNPs ) in transcription factor binding sites ( TFBSs ) may affect the binding of transcription factors , lead to differences in gene expression and phenotypes and therefore affect susceptibility to environmental exposure .
	manualset3
137551	4	407106	5	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Single nucleotide polymorphisms ( SNPs ) in transcription factor binding sites ( TFBSs ) may affect the binding of transcription factors , lead to differences in gene expression and phenotypes and therefore affect susceptibility to environmental exposure .
	manualset3
137552	5	407106	5	NULL	NULL	0	NULL	transcription factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Single nucleotide polymorphisms ( SNPs ) in transcription factor binding sites ( TFBSs ) may affect the binding of transcription factors , lead to differences in gene expression and phenotypes and therefore affect susceptibility to environmental exposure .
	manualset3
137553	6	407106	5	NULL	NULL	0	NULL	differences 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Single nucleotide polymorphisms ( SNPs ) in transcription factor binding sites ( TFBSs ) may affect the binding of transcription factors , lead to differences in gene expression and phenotypes and therefore affect susceptibility to environmental exposure .
	manualset3
137554	7	407106	5	NULL	NULL	0	NULL	gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Single nucleotide polymorphisms ( SNPs ) in transcription factor binding sites ( TFBSs ) may affect the binding of transcription factors , lead to differences in gene expression and phenotypes and therefore affect susceptibility to environmental exposure .
	manualset3
137555	8	407106	5	NULL	NULL	0	NULL	phenotypes 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Single nucleotide polymorphisms ( SNPs ) in transcription factor binding sites ( TFBSs ) may affect the binding of transcription factors , lead to differences in gene expression and phenotypes and therefore affect susceptibility to environmental exposure .
	manualset3
137557	10	407106	5	NULL	NULL	0	NULL	susceptibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Single nucleotide polymorphisms ( SNPs ) in transcription factor binding sites ( TFBSs ) may affect the binding of transcription factors , lead to differences in gene expression and phenotypes and therefore affect susceptibility to environmental exposure .
	manualset3
137558	11	407106	5	NULL	NULL	0	NULL	environmental exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Single nucleotide polymorphisms ( SNPs ) in transcription factor binding sites ( TFBSs ) may affect the binding of transcription factors , lead to differences in gene expression and phenotypes and therefore affect susceptibility to environmental exposure .
	manualset3
137559	1	407107	5	NULL	NULL	0	NULL	Single patient tissue microarrays ( TMAs ) 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Single patient tissue microarrays ( TMAs ) were constructed from archived PBC and post-mortem MBCs .
	manualset3
137560	2	407107	5	NULL	NULL	0	NULL	archived PBC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Single patient tissue microarrays ( TMAs ) were constructed from archived PBC and post-mortem MBCs .
	manualset3
137561	3	407107	5	NULL	NULL	0	NULL	post-mortem MBCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Single patient tissue microarrays ( TMAs ) were constructed from archived PBC and post-mortem MBCs .
	manualset3
137562	1	407108	5	NULL	NULL	0	NULL	polyprenol and dolichol isolation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Single polyprenol and dolichol isolation by semipreparative high-performance liquid chromatography technique .
	manualset3
137563	2	407108	5	NULL	NULL	0	NULL	semipreparative high-performance liquid chromatography technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Single polyprenol and dolichol isolation by semipreparative high-performance liquid chromatography technique .
	manualset3
137564	1	407109	5	NULL	NULL	0	NULL	pulse stimuli 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Single pulse stimuli were delivered to the Schaffer collaterals in the in vitro hippocampal slice preparation .
	manualset3
137565	2	407109	5	NULL	NULL	0	NULL	Schaffer collaterals 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Single pulse stimuli were delivered to the Schaffer collaterals in the in vitro hippocampal slice preparation .
	manualset3
137566	3	407109	5	NULL	NULL	0	NULL	in vitro hippocampal slice preparation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Single pulse stimuli were delivered to the Schaffer collaterals in the in vitro hippocampal slice preparation .
	manualset3
137567	1	407110	5	NULL	NULL	0	NULL	Single units 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Single units excited by microinjection of atrial natriuretic peptide into the caudal nucleus tractus solitarii were also excited by activation of arterial baroreceptors and inhibited by baroreceptor unloading .
	manualset3
137568	2	407110	5	NULL	NULL	0	NULL	microinjection 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Single units excited by microinjection of atrial natriuretic peptide into the caudal nucleus tractus solitarii were also excited by activation of arterial baroreceptors and inhibited by baroreceptor unloading .
	manualset3
137569	3	407110	5	NULL	NULL	0	NULL	atrial natriuretic peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Single units excited by microinjection of atrial natriuretic peptide into the caudal nucleus tractus solitarii were also excited by activation of arterial baroreceptors and inhibited by baroreceptor unloading .
	manualset3
137570	4	407110	5	NULL	NULL	0	NULL	caudal nucleus tractus solitarii	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Single units excited by microinjection of atrial natriuretic peptide into the caudal nucleus tractus solitarii were also excited by activation of arterial baroreceptors and inhibited by baroreceptor unloading .
	manualset3
137571	5	407110	5	NULL	NULL	0	NULL	activation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Single units excited by microinjection of atrial natriuretic peptide into the caudal nucleus tractus solitarii were also excited by activation of arterial baroreceptors and inhibited by baroreceptor unloading .
	manualset3
137572	6	407110	5	NULL	NULL	0	NULL	arterial baroreceptors	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Single units excited by microinjection of atrial natriuretic peptide into the caudal nucleus tractus solitarii were also excited by activation of arterial baroreceptors and inhibited by baroreceptor unloading .
	manualset3
137573	7	407110	5	NULL	NULL	0	NULL	baroreceptor unloading	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Single units excited by microinjection of atrial natriuretic peptide into the caudal nucleus tractus solitarii were also excited by activation of arterial baroreceptors and inhibited by baroreceptor unloading .
	manualset3
137574	1	407111	5	NULL	NULL	0	NULL	Singlet molecular oxygen	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Singlet molecular oxygen induced mutagenicity in a mammalian SV40-based shuttle vector .
	manualset3
137575	2	407111	5	NULL	NULL	0	NULL	mutagenicity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Singlet molecular oxygen induced mutagenicity in a mammalian SV40-based shuttle vector .
	manualset3
137576	3	407111	5	NULL	NULL	0	NULL	mammalian SV40-based shuttle vector	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Singlet molecular oxygen induced mutagenicity in a mammalian SV40-based shuttle vector .
	manualset3
137577	1	407112	5	NULL	NULL	0	NULL	Sinus cycle length ( SCL )	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Sinus cycle length ( SCL ) shortened significantly after PAB in both groups .
	manualset3
137578	2	407112	5	NULL	NULL	0	NULL	PAB 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sinus cycle length ( SCL ) shortened significantly after PAB in both groups .
	manualset3
137579	3	407112	5	NULL	NULL	0	NULL	groups 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sinus cycle length ( SCL ) shortened significantly after PAB in both groups .
	manualset3
137580	1	407113	5	NULL	NULL	0	NULL	Sir3 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sir3 is closely related to the origin recognition complex 1 subunit and consists of an N-terminal bromo-adjacent homology ( BAH ) domain and a C-terminal AAA ( + ) ATPase-like domain .
	manualset3
137581	2	407113	5	NULL	NULL	0	NULL	origin recognition complex 1 subunit 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sir3 is closely related to the origin recognition complex 1 subunit and consists of an N-terminal bromo-adjacent homology ( BAH ) domain and a C-terminal AAA ( + ) ATPase-like domain .
	manualset3
137582	3	407113	5	NULL	NULL	0	NULL	N-terminal bromo-adjacent homology ( BAH ) domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sir3 is closely related to the origin recognition complex 1 subunit and consists of an N-terminal bromo-adjacent homology ( BAH ) domain and a C-terminal AAA ( + ) ATPase-like domain .
	manualset3
137583	4	407113	5	NULL	NULL	0	NULL	 C-terminal AAA ( + ) ATPase-like domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sir3 is closely related to the origin recognition complex 1 subunit and consists of an N-terminal bromo-adjacent homology ( BAH ) domain and a C-terminal AAA ( + ) ATPase-like domain .
	manualset3
137584	1	407114	5	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of resident characteristics were not described well by case-mix measures based only on service use , suggesting the need to modify such groups using additional sources of input .
	manualset3
137585	2	407114	5	NULL	NULL	0	NULL	resident characteristics 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of resident characteristics were not described well by case-mix measures based only on service use , suggesting the need to modify such groups using additional sources of input .
	manualset3
137586	3	407114	5	NULL	NULL	0	NULL	case-mix measures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of resident characteristics were not described well by case-mix measures based only on service use , suggesting the need to modify such groups using additional sources of input .
	manualset3
137587	4	407114	5	NULL	NULL	0	NULL	service use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of resident characteristics were not described well by case-mix measures based only on service use , suggesting the need to modify such groups using additional sources of input .
	manualset3
137588	5	407114	5	NULL	NULL	0	NULL	need 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of resident characteristics were not described well by case-mix measures based only on service use , suggesting the need to modify such groups using additional sources of input .
	manualset3
137590	7	407114	5	NULL	NULL	0	NULL	groups 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of resident characteristics were not described well by case-mix measures based only on service use , suggesting the need to modify such groups using additional sources of input .
	manualset3
137591	8	407114	5	NULL	NULL	0	NULL	additional sources	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of resident characteristics were not described well by case-mix measures based only on service use , suggesting the need to modify such groups using additional sources of input .
	manualset3
137592	9	407114	5	NULL	NULL	0	NULL	input 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of resident characteristics were not described well by case-mix measures based only on service use , suggesting the need to modify such groups using additional sources of input .
	manualset3
137593	1	407115	5	NULL	NULL	0	NULL	ister chromatid exchange ( SCE ) frequency 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sister chromatid exchange ( SCE ) frequency in lymphocytes of patients with colorectal carcinoma treated with razoxane .
	manualset3
137594	2	407115	5	NULL	NULL	0	NULL	lymphocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Sister chromatid exchange ( SCE ) frequency in lymphocytes of patients with colorectal carcinoma treated with razoxane .
	manualset3
137595	3	407115	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sister chromatid exchange ( SCE ) frequency in lymphocytes of patients with colorectal carcinoma treated with razoxane .
	manualset3
137596	4	407115	5	NULL	NULL	0	NULL	colorectal carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Sister chromatid exchange ( SCE ) frequency in lymphocytes of patients with colorectal carcinoma treated with razoxane .
	manualset3
137597	5	407115	5	NULL	NULL	0	NULL	razoxane 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Sister chromatid exchange ( SCE ) frequency in lymphocytes of patients with colorectal carcinoma treated with razoxane .
	manualset3
137598	1	407116	5	NULL	NULL	0	NULL	Site-directed mutagenesis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Site-directed mutagenesis confirmed that all six extracellular asparagines are N-glycosylated and that the Ser/Thr/Pro cluster in the `` stalk '' domain juxtaposed to the cysteine-rich domains ( CRDs ) is a major site for the likely mucine-type of O-glycosylation .
	manualset3
137599	2	407116	5	NULL	NULL	0	NULL	six 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Site-directed mutagenesis confirmed that all six extracellular asparagines are N-glycosylated and that the Ser/Thr/Pro cluster in the `` stalk '' domain juxtaposed to the cysteine-rich domains ( CRDs ) is a major site for the likely mucine-type of O-glycosylation .
	manualset3
137600	3	407116	5	NULL	NULL	0	NULL	extracellular asparagines 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Site-directed mutagenesis confirmed that all six extracellular asparagines are N-glycosylated and that the Ser/Thr/Pro cluster in the `` stalk '' domain juxtaposed to the cysteine-rich domains ( CRDs ) is a major site for the likely mucine-type of O-glycosylation .
	manualset3
137601	4	407116	5	NULL	NULL	0	NULL	Ser/Thr/Pro cluster	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Site-directed mutagenesis confirmed that all six extracellular asparagines are N-glycosylated and that the Ser/Thr/Pro cluster in the `` stalk '' domain juxtaposed to the cysteine-rich domains ( CRDs ) is a major site for the likely mucine-type of O-glycosylation .
	manualset3
137602	5	407116	5	NULL	NULL	0	NULL	 `` stalk '' domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Site-directed mutagenesis confirmed that all six extracellular asparagines are N-glycosylated and that the Ser/Thr/Pro cluster in the `` stalk '' domain juxtaposed to the cysteine-rich domains ( CRDs ) is a major site for the likely mucine-type of O-glycosylation .
	manualset3
137603	6	407116	5	NULL	NULL	0	NULL	cysteine-rich domains ( CRDs )	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Site-directed mutagenesis confirmed that all six extracellular asparagines are N-glycosylated and that the Ser/Thr/Pro cluster in the `` stalk '' domain juxtaposed to the cysteine-rich domains ( CRDs ) is a major site for the likely mucine-type of O-glycosylation .
	manualset3
137604	7	407116	5	NULL	NULL	0	NULL	site 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Site-directed mutagenesis confirmed that all six extracellular asparagines are N-glycosylated and that the Ser/Thr/Pro cluster in the `` stalk '' domain juxtaposed to the cysteine-rich domains ( CRDs ) is a major site for the likely mucine-type of O-glycosylation .
	manualset3
137605	8	407116	5	NULL	NULL	0	NULL	mucine-type of O-glycosylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Site-directed mutagenesis confirmed that all six extracellular asparagines are N-glycosylated and that the Ser/Thr/Pro cluster in the `` stalk '' domain juxtaposed to the cysteine-rich domains ( CRDs ) is a major site for the likely mucine-type of O-glycosylation .
	manualset3
137606	1	407117	5	NULL	NULL	0	NULL	Site-directed mutagenesis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Site-directed mutagenesis has proved to be a most useful tool for the identification of the intermediates involved and the resulting nature of the compound I formed .
	manualset3
137607	2	407117	5	NULL	NULL	0	NULL	useful tool	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Site-directed mutagenesis has proved to be a most useful tool for the identification of the intermediates involved and the resulting nature of the compound I formed .
	manualset3
137608	3	407117	5	NULL	NULL	0	NULL	identification 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Site-directed mutagenesis has proved to be a most useful tool for the identification of the intermediates involved and the resulting nature of the compound I formed .
	manualset3
137609	4	407117	5	NULL	NULL	0	NULL	intermediates 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Site-directed mutagenesis has proved to be a most useful tool for the identification of the intermediates involved and the resulting nature of the compound I formed .
	manualset3
137610	5	407117	5	NULL	NULL	0	NULL	resulting nature	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Site-directed mutagenesis has proved to be a most useful tool for the identification of the intermediates involved and the resulting nature of the compound I formed .
	manualset3
137611	6	407117	5	NULL	NULL	NULL	NULL	compound I	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Site-directed mutagenesis has proved to be a most useful tool for the identification of the intermediates involved and the resulting nature of the compound I formed .
	manualset3
137612	1	407118	5	NULL	NULL	0	NULL	Site-directed mutagenesis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Site-directed mutagenesis of cysteine residues of Luciola mingrelica firefly luciferase .
	manualset3
137613	2	407118	5	NULL	NULL	0	NULL	cysteine residues 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Site-directed mutagenesis of cysteine residues of Luciola mingrelica firefly luciferase .
	manualset3
137614	3	407118	5	NULL	NULL	0	NULL	Luciola mingrelica firefly luciferase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Site-directed mutagenesis of cysteine residues of Luciola mingrelica firefly luciferase .
	manualset3
137615	1	407119	5	NULL	NULL	0	NULL	Site-directed mutagenesis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Site-directed mutagenesis was used to produce 6 mutant Fpg proteins with Cys -- ) Gly mutations .
	manualset3
137616	2	407119	5	NULL	NULL	0	NULL	6	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Site-directed mutagenesis was used to produce 6 mutant Fpg proteins with Cys -- ) Gly mutations .
	manualset3
137617	3	407119	5	NULL	NULL	0	NULL	mutant Fpg proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Site-directed mutagenesis was used to produce 6 mutant Fpg proteins with Cys -- ) Gly mutations .
	manualset3
137618	4	407119	5	NULL	NULL	0	NULL	Cys -- ) Gly mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Site-directed mutagenesis was used to produce 6 mutant Fpg proteins with Cys -- ) Gly mutations .
	manualset3
137619	1	407120	5	NULL	NULL	0	NULL	Situations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Situations may arise in which untreated disease , acute infections , failing restorations , or trauma result in pain or discomfort .
	manualset3
137620	2	407120	5	NULL	NULL	0	NULL	untreated disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Situations may arise in which untreated disease , acute infections , failing restorations , or trauma result in pain or discomfort .
	manualset3
137621	3	407120	5	NULL	NULL	0	NULL	acute infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Situations may arise in which untreated disease , acute infections , failing restorations , or trauma result in pain or discomfort .
	manualset3
137622	4	407120	5	NULL	NULL	0	NULL	failing restorations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Situations may arise in which untreated disease , acute infections , failing restorations , or trauma result in pain or discomfort .
	manualset3
137623	5	407120	5	NULL	NULL	0	NULL	trauma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Situations may arise in which untreated disease , acute infections , failing restorations , or trauma result in pain or discomfort .
	manualset3
137624	6	407120	5	NULL	NULL	0	NULL	pain 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Situations may arise in which untreated disease , acute infections , failing restorations , or trauma result in pain or discomfort .
	manualset3
137625	7	407120	5	NULL	NULL	0	NULL	discomfort 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Situations may arise in which untreated disease , acute infections , failing restorations , or trauma result in pain or discomfort .
	manualset3
137626	1	407121	5	NULL	NULL	0	NULL	Six-dimensional quantum dynamical calculations 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Six-dimensional quantum dynamical calculations are reported for the dissociative chemisorption of ( v = 0 , 1 , j = 0 ) H ( 2 ) on Cu ( 100 ) , and for rovibrationally inelastic scattering of ( v = 1 , j = 1 ) H ( 2 ) from Cu ( 100 ) .
	manualset3
137627	2	407121	5	NULL	NULL	0	NULL	dissociative chemisorption 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Six-dimensional quantum dynamical calculations are reported for the dissociative chemisorption of ( v = 0 , 1 , j = 0 ) H ( 2 ) on Cu ( 100 ) , and for rovibrationally inelastic scattering of ( v = 1 , j = 1 ) H ( 2 ) from Cu ( 100 ) .
	manualset3
137628	3	407121	5	NULL	NULL	0	NULL	 ( v = 0 , 1 , j = 0 ) H ( 2 )	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Six-dimensional quantum dynamical calculations are reported for the dissociative chemisorption of ( v = 0 , 1 , j = 0 ) H ( 2 ) on Cu ( 100 ) , and for rovibrationally inelastic scattering of ( v = 1 , j = 1 ) H ( 2 ) from Cu ( 100 ) .
	manualset3
137629	4	407121	5	NULL	NULL	0	NULL	Cu ( 100 )	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Six-dimensional quantum dynamical calculations are reported for the dissociative chemisorption of ( v = 0 , 1 , j = 0 ) H ( 2 ) on Cu ( 100 ) , and for rovibrationally inelastic scattering of ( v = 1 , j = 1 ) H ( 2 ) from Cu ( 100 ) .
	manualset3
137630	5	407121	5	NULL	NULL	0	NULL	rovibrationally inelastic scattering	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Six-dimensional quantum dynamical calculations are reported for the dissociative chemisorption of ( v = 0 , 1 , j = 0 ) H ( 2 ) on Cu ( 100 ) , and for rovibrationally inelastic scattering of ( v = 1 , j = 1 ) H ( 2 ) from Cu ( 100 ) .
	manualset3
137631	6	407121	5	NULL	NULL	0	NULL	( v = 1 , j = 1 ) H ( 2 )	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Six-dimensional quantum dynamical calculations are reported for the dissociative chemisorption of ( v = 0 , 1 , j = 0 ) H ( 2 ) on Cu ( 100 ) , and for rovibrationally inelastic scattering of ( v = 1 , j = 1 ) H ( 2 ) from Cu ( 100 ) .
	manualset3
137632	7	407121	5	NULL	NULL	0	NULL	Cu ( 100 )	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Six-dimensional quantum dynamical calculations are reported for the dissociative chemisorption of ( v = 0 , 1 , j = 0 ) H ( 2 ) on Cu ( 100 ) , and for rovibrationally inelastic scattering of ( v = 1 , j = 1 ) H ( 2 ) from Cu ( 100 ) .
	manualset3
137633	1	407122	5	NULL	NULL	0	NULL	Six 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six ( all renal ) patients received conventional immunosuppressive therapy ( CIT ) , four received cyclosporin A ( CsA ) ( one cardiac , one hepatic , two renal ) , and one received CIT for his first transplant and CsA for his second transplant ( both renal ) .
	manualset3
137634	2	407122	5	NULL	NULL	0	NULL	( all renal ) patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Six ( all renal ) patients received conventional immunosuppressive therapy ( CIT ) , four received cyclosporin A ( CsA ) ( one cardiac , one hepatic , two renal ) , and one received CIT for his first transplant and CsA for his second transplant ( both renal ) .
	manualset3
137635	3	407122	5	NULL	NULL	0	NULL	conventional immunosuppressive therapy ( CIT )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Six ( all renal ) patients received conventional immunosuppressive therapy ( CIT ) , four received cyclosporin A ( CsA ) ( one cardiac , one hepatic , two renal ) , and one received CIT for his first transplant and CsA for his second transplant ( both renal ) .
	manualset3
137636	4	407122	5	NULL	NULL	0	NULL	four 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six ( all renal ) patients received conventional immunosuppressive therapy ( CIT ) , four received cyclosporin A ( CsA ) ( one cardiac , one hepatic , two renal ) , and one received CIT for his first transplant and CsA for his second transplant ( both renal ) .
	manualset3
137637	5	407122	5	NULL	NULL	0	NULL	cyclosporin A ( CsA )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Six ( all renal ) patients received conventional immunosuppressive therapy ( CIT ) , four received cyclosporin A ( CsA ) ( one cardiac , one hepatic , two renal ) , and one received CIT for his first transplant and CsA for his second transplant ( both renal ) .
	manualset3
137638	6	407122	5	NULL	NULL	0	NULL	one cardiac 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six ( all renal ) patients received conventional immunosuppressive therapy ( CIT ) , four received cyclosporin A ( CsA ) ( one cardiac , one hepatic , two renal ) , and one received CIT for his first transplant and CsA for his second transplant ( both renal ) .
	manualset3
137639	7	407122	5	NULL	NULL	0	NULL	one hepatic	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six ( all renal ) patients received conventional immunosuppressive therapy ( CIT ) , four received cyclosporin A ( CsA ) ( one cardiac , one hepatic , two renal ) , and one received CIT for his first transplant and CsA for his second transplant ( both renal ) .
	manualset3
137640	8	407122	5	NULL	NULL	0	NULL	two renal	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six ( all renal ) patients received conventional immunosuppressive therapy ( CIT ) , four received cyclosporin A ( CsA ) ( one cardiac , one hepatic , two renal ) , and one received CIT for his first transplant and CsA for his second transplant ( both renal ) .
	manualset3
137641	9	407122	5	NULL	NULL	0	NULL	one 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six ( all renal ) patients received conventional immunosuppressive therapy ( CIT ) , four received cyclosporin A ( CsA ) ( one cardiac , one hepatic , two renal ) , and one received CIT for his first transplant and CsA for his second transplant ( both renal ) .
	manualset3
137642	10	407122	5	NULL	NULL	0	NULL	CIT 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Six ( all renal ) patients received conventional immunosuppressive therapy ( CIT ) , four received cyclosporin A ( CsA ) ( one cardiac , one hepatic , two renal ) , and one received CIT for his first transplant and CsA for his second transplant ( both renal ) .
	manualset3
137643	11	407122	5	NULL	NULL	0	NULL	 first transplant 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six ( all renal ) patients received conventional immunosuppressive therapy ( CIT ) , four received cyclosporin A ( CsA ) ( one cardiac , one hepatic , two renal ) , and one received CIT for his first transplant and CsA for his second transplant ( both renal ) .
	manualset3
137644	12	407122	5	NULL	NULL	0	NULL	CsA 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Six ( all renal ) patients received conventional immunosuppressive therapy ( CIT ) , four received cyclosporin A ( CsA ) ( one cardiac , one hepatic , two renal ) , and one received CIT for his first transplant and CsA for his second transplant ( both renal ) .
	manualset3
137645	13	407122	5	NULL	NULL	0	NULL	second transplant	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six ( all renal ) patients received conventional immunosuppressive therapy ( CIT ) , four received cyclosporin A ( CsA ) ( one cardiac , one hepatic , two renal ) , and one received CIT for his first transplant and CsA for his second transplant ( both renal ) .
	manualset3
137646	1	407123	5	NULL	NULL	0	NULL	Six hr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Six and 24 hr after the injection of cadmium sulfate , the accumulation of maternal hepatic cadmium increased and that in the decidua , including embryos , decreased after pretreatment with bismuth nitrate .
	manualset3
137647	2	407123	5	NULL	NULL	0	NULL	 24 hr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Six and 24 hr after the injection of cadmium sulfate , the accumulation of maternal hepatic cadmium increased and that in the decidua , including embryos , decreased after pretreatment with bismuth nitrate .
	manualset3
137648	3	407123	5	NULL	NULL	0	NULL	injection 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Six and 24 hr after the injection of cadmium sulfate , the accumulation of maternal hepatic cadmium increased and that in the decidua , including embryos , decreased after pretreatment with bismuth nitrate .
	manualset3
137649	4	407123	5	NULL	NULL	0	NULL	cadmium sulfate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Six and 24 hr after the injection of cadmium sulfate , the accumulation of maternal hepatic cadmium increased and that in the decidua , including embryos , decreased after pretreatment with bismuth nitrate .
	manualset3
137650	5	407123	5	NULL	NULL	0	NULL	accumulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Six and 24 hr after the injection of cadmium sulfate , the accumulation of maternal hepatic cadmium increased and that in the decidua , including embryos , decreased after pretreatment with bismuth nitrate .
	manualset3
137651	6	407123	5	NULL	NULL	0	NULL	maternal hepatic cadmium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Six and 24 hr after the injection of cadmium sulfate , the accumulation of maternal hepatic cadmium increased and that in the decidua , including embryos , decreased after pretreatment with bismuth nitrate .
	manualset3
137652	7	407123	5	NULL	NULL	0	NULL	decidua 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Six and 24 hr after the injection of cadmium sulfate , the accumulation of maternal hepatic cadmium increased and that in the decidua , including embryos , decreased after pretreatment with bismuth nitrate .
	manualset3
137653	8	407123	5	NULL	NULL	0	NULL	embryos 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Six and 24 hr after the injection of cadmium sulfate , the accumulation of maternal hepatic cadmium increased and that in the decidua , including embryos , decreased after pretreatment with bismuth nitrate .
	manualset3
137654	9	407123	5	NULL	NULL	NULL	NULL	pretreatment 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Six and 24 hr after the injection of cadmium sulfate , the accumulation of maternal hepatic cadmium increased and that in the decidua , including embryos , decreased after pretreatment with bismuth nitrate .
	manualset3
137655	10	407123	5	NULL	NULL	0	NULL	bismuth nitrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Six and 24 hr after the injection of cadmium sulfate , the accumulation of maternal hepatic cadmium increased and that in the decidua , including embryos , decreased after pretreatment with bismuth nitrate .
	manualset3
137656	1	407124	5	NULL	NULL	0	NULL	Six cases	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six cases of Scopulariopsis onychomycosis , including four patients with onychomycosis exclusively caused by Scopulariopsis brevicaulis and two patients with a mixed nail infection ( S. brevicaulis + Tricophyton rubrum and S. brevicaulis + T. interdigitale ) , are reported .
	manualset3
137657	2	407124	5	NULL	NULL	0	NULL	Scopulariopsis onychomycosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Six cases of Scopulariopsis onychomycosis , including four patients with onychomycosis exclusively caused by Scopulariopsis brevicaulis and two patients with a mixed nail infection ( S. brevicaulis + Tricophyton rubrum and S. brevicaulis + T. interdigitale ) , are reported .
	manualset3
137658	3	407124	5	NULL	NULL	0	NULL	four patients 	meas												NULL		0	NULL	NULL	NULL	NULL	NULL	Six cases of Scopulariopsis onychomycosis , including four patients with onychomycosis exclusively caused by Scopulariopsis brevicaulis and two patients with a mixed nail infection ( S. brevicaulis + Tricophyton rubrum and S. brevicaulis + T. interdigitale ) , are reported .
	manualset3
137659	4	407124	5	NULL	NULL	0	NULL	onychomycosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Six cases of Scopulariopsis onychomycosis , including four patients with onychomycosis exclusively caused by Scopulariopsis brevicaulis and two patients with a mixed nail infection ( S. brevicaulis + Tricophyton rubrum and S. brevicaulis + T. interdigitale ) , are reported .
	manualset3
137660	5	407124	5	NULL	NULL	0	NULL	Scopulariopsis brevicaulis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Six cases of Scopulariopsis onychomycosis , including four patients with onychomycosis exclusively caused by Scopulariopsis brevicaulis and two patients with a mixed nail infection ( S. brevicaulis + Tricophyton rubrum and S. brevicaulis + T. interdigitale ) , are reported .
	manualset3
137661	6	407124	5	NULL	NULL	0	NULL	two patients	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six cases of Scopulariopsis onychomycosis , including four patients with onychomycosis exclusively caused by Scopulariopsis brevicaulis and two patients with a mixed nail infection ( S. brevicaulis + Tricophyton rubrum and S. brevicaulis + T. interdigitale ) , are reported .
	manualset3
137662	7	407124	5	NULL	NULL	0	NULL	mixed nail infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Six cases of Scopulariopsis onychomycosis , including four patients with onychomycosis exclusively caused by Scopulariopsis brevicaulis and two patients with a mixed nail infection ( S. brevicaulis + Tricophyton rubrum and S. brevicaulis + T. interdigitale ) , are reported .
	manualset3
137663	8	407124	5	NULL	NULL	0	NULL	S. brevicaulis + Tricophyton rubrum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Six cases of Scopulariopsis onychomycosis , including four patients with onychomycosis exclusively caused by Scopulariopsis brevicaulis and two patients with a mixed nail infection ( S. brevicaulis + Tricophyton rubrum and S. brevicaulis + T. interdigitale ) , are reported .
	manualset3
137664	9	407124	5	NULL	NULL	0	NULL	S. brevicaulis + T. interdigitale	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Six cases of Scopulariopsis onychomycosis , including four patients with onychomycosis exclusively caused by Scopulariopsis brevicaulis and two patients with a mixed nail infection ( S. brevicaulis + Tricophyton rubrum and S. brevicaulis + T. interdigitale ) , are reported .
	manualset3
137665	1	407125	5	NULL	NULL	0	NULL	Six devices 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six devices were replaced because of excessive residual leaks , three for premature lock release , and two for improper seating of the device .
	manualset3
137666	2	407125	5	NULL	NULL	0	NULL	excessive residual leaks	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Six devices were replaced because of excessive residual leaks , three for premature lock release , and two for improper seating of the device .
	manualset3
137667	3	407125	5	NULL	NULL	0	NULL	three 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six devices were replaced because of excessive residual leaks , three for premature lock release , and two for improper seating of the device .
	manualset3
137668	4	407125	5	NULL	NULL	0	NULL	premature lock release	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Six devices were replaced because of excessive residual leaks , three for premature lock release , and two for improper seating of the device .
	manualset3
137669	5	407125	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six devices were replaced because of excessive residual leaks , three for premature lock release , and two for improper seating of the device .
	manualset3
137670	6	407125	5	NULL	NULL	0	NULL	improper seating 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Six devices were replaced because of excessive residual leaks , three for premature lock release , and two for improper seating of the device .
	manualset3
137671	7	407125	5	NULL	NULL	0	NULL	device 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Six devices were replaced because of excessive residual leaks , three for premature lock release , and two for improper seating of the device .
	manualset3
137672	1	407126	5	NULL	NULL	0	NULL	Six feet 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six feet did not have radiographic union , yet only two lost correction requiring repeated surgery .
	manualset3
137673	2	407126	5	NULL	NULL	0	NULL	radiographic union	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Six feet did not have radiographic union , yet only two lost correction requiring repeated surgery .
	manualset3
137674	3	407126	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six feet did not have radiographic union , yet only two lost correction requiring repeated surgery .
	manualset3
137675	4	407126	5	NULL	NULL	0	NULL	correction 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Six feet did not have radiographic union , yet only two lost correction requiring repeated surgery .
	manualset3
137676	5	407126	5	NULL	NULL	0	NULL	repeated surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Six feet did not have radiographic union , yet only two lost correction requiring repeated surgery .
	manualset3
137677	1	407127	5	NULL	NULL	0	NULL	Six implants	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six implants were milled with a diamond bur while the other six implants remained intact .
	manualset3
137678	2	407127	5	NULL	NULL	0	NULL	diamond bur	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Six implants were milled with a diamond bur while the other six implants remained intact .
	manualset3
137679	3	407127	5	NULL	NULL	0	NULL	six implants	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six implants were milled with a diamond bur while the other six implants remained intact .
	manualset3
137680	1	407128	5	NULL	NULL	0	NULL	Six monoclonal antibodies	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six monoclonal antibodies to human pancreatic cancer antigens .
	manualset3
137681	2	407128	5	NULL	NULL	0	NULL	human pancreatic cancer antigens	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Six monoclonal antibodies to human pancreatic cancer antigens .
	manualset3
137682	1	407129	5	NULL	NULL	0	NULL	Six novel agents 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six novel agents - sunitinib , sorafenib , temsirolimus , everolimus , bevacizumab ( used in combination with interferon ) , and pazopanib ( Votrient ) - have been approved for the treatment of metastatic RCC .
	manualset3
137683	2	407129	5	NULL	NULL	0	NULL	sunitinib 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Six novel agents - sunitinib , sorafenib , temsirolimus , everolimus , bevacizumab ( used in combination with interferon ) , and pazopanib ( Votrient ) - have been approved for the treatment of metastatic RCC .
	manualset3
137684	3	407129	5	NULL	NULL	0	NULL	sorafenib 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Six novel agents - sunitinib , sorafenib , temsirolimus , everolimus , bevacizumab ( used in combination with interferon ) , and pazopanib ( Votrient ) - have been approved for the treatment of metastatic RCC .
	manualset3
137685	4	407129	5	NULL	NULL	0	NULL	temsirolimus 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Six novel agents - sunitinib , sorafenib , temsirolimus , everolimus , bevacizumab ( used in combination with interferon ) , and pazopanib ( Votrient ) - have been approved for the treatment of metastatic RCC .
	manualset3
137686	5	407129	5	NULL	NULL	0	NULL	everolimus 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Six novel agents - sunitinib , sorafenib , temsirolimus , everolimus , bevacizumab ( used in combination with interferon ) , and pazopanib ( Votrient ) - have been approved for the treatment of metastatic RCC .
	manualset3
137687	6	407129	5	NULL	NULL	0	NULL	bevacizumab 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Six novel agents - sunitinib , sorafenib , temsirolimus , everolimus , bevacizumab ( used in combination with interferon ) , and pazopanib ( Votrient ) - have been approved for the treatment of metastatic RCC .
	manualset3
137688	7	407129	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Six novel agents - sunitinib , sorafenib , temsirolimus , everolimus , bevacizumab ( used in combination with interferon ) , and pazopanib ( Votrient ) - have been approved for the treatment of metastatic RCC .
	manualset3
137689	8	407129	5	NULL	NULL	0	NULL	interferon 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Six novel agents - sunitinib , sorafenib , temsirolimus , everolimus , bevacizumab ( used in combination with interferon ) , and pazopanib ( Votrient ) - have been approved for the treatment of metastatic RCC .
	manualset3
137690	9	407129	5	NULL	NULL	0	NULL	pazopanib ( Votrient ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Six novel agents - sunitinib , sorafenib , temsirolimus , everolimus , bevacizumab ( used in combination with interferon ) , and pazopanib ( Votrient ) - have been approved for the treatment of metastatic RCC .
	manualset3
137691	10	407129	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Six novel agents - sunitinib , sorafenib , temsirolimus , everolimus , bevacizumab ( used in combination with interferon ) , and pazopanib ( Votrient ) - have been approved for the treatment of metastatic RCC .
	manualset3
137692	11	407129	5	NULL	NULL	0	NULL	metastatic RCC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Six novel agents - sunitinib , sorafenib , temsirolimus , everolimus , bevacizumab ( used in combination with interferon ) , and pazopanib ( Votrient ) - have been approved for the treatment of metastatic RCC .
	manualset3
137693	1	407130	5	NULL	NULL	0	NULL	Six of 102 persons	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six of 102 persons tested in both months showed at least a fourfold rise in titer of antibodies to B. microti ( an incidence of 5.9 % for the season ) .
	manualset3
137694	2	407130	5	NULL	NULL	0	NULL	months 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Six of 102 persons tested in both months showed at least a fourfold rise in titer of antibodies to B. microti ( an incidence of 5.9 % for the season ) .
	manualset3
137695	3	407130	5	NULL	NULL	0	NULL	fourfold rise	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six of 102 persons tested in both months showed at least a fourfold rise in titer of antibodies to B. microti ( an incidence of 5.9 % for the season ) .
	manualset3
137696	4	407130	5	NULL	NULL	0	NULL	titer 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Six of 102 persons tested in both months showed at least a fourfold rise in titer of antibodies to B. microti ( an incidence of 5.9 % for the season ) .
	manualset3
137697	5	407130	5	NULL	NULL	0	NULL	antibodies to B. microti 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Six of 102 persons tested in both months showed at least a fourfold rise in titer of antibodies to B. microti ( an incidence of 5.9 % for the season ) .
	manualset3
137698	6	407130	5	NULL	NULL	0	NULL	incidence 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Six of 102 persons tested in both months showed at least a fourfold rise in titer of antibodies to B. microti ( an incidence of 5.9 % for the season ) .
	manualset3
137699	7	407130	5	NULL	NULL	0	NULL	 5.9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six of 102 persons tested in both months showed at least a fourfold rise in titer of antibodies to B. microti ( an incidence of 5.9 % for the season ) .
	manualset3
137700	8	407130	5	NULL	NULL	0	NULL	season 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Six of 102 persons tested in both months showed at least a fourfold rise in titer of antibodies to B. microti ( an incidence of 5.9 % for the season ) .
	manualset3
137701	1	407131	5	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of studies suggest that similar pathophysiologic mechanisms are responsible for development and progression of calcification of atherosclerotic plaque and bone formation .
	manualset3
137702	2	407131	5	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of studies suggest that similar pathophysiologic mechanisms are responsible for development and progression of calcification of atherosclerotic plaque and bone formation .
	manualset3
137703	3	407131	5	NULL	NULL	0	NULL	pathophysiologic mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of studies suggest that similar pathophysiologic mechanisms are responsible for development and progression of calcification of atherosclerotic plaque and bone formation .
	manualset3
137704	4	407131	5	NULL	NULL	NULL	NULL	development 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A number of studies suggest that similar pathophysiologic mechanisms are responsible for development and progression of calcification of atherosclerotic plaque and bone formation .
	manualset3
137705	5	407131	5	NULL	NULL	0	NULL	progression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of studies suggest that similar pathophysiologic mechanisms are responsible for development and progression of calcification of atherosclerotic plaque and bone formation .
	manualset3
137706	6	407131	5	NULL	NULL	0	NULL	calcification 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of studies suggest that similar pathophysiologic mechanisms are responsible for development and progression of calcification of atherosclerotic plaque and bone formation .
	manualset3
137707	7	407131	5	NULL	NULL	0	NULL	atherosclerotic plaque 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of studies suggest that similar pathophysiologic mechanisms are responsible for development and progression of calcification of atherosclerotic plaque and bone formation .
	manualset3
137708	8	407131	5	NULL	NULL	0	NULL	bone formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of studies suggest that similar pathophysiologic mechanisms are responsible for development and progression of calcification of atherosclerotic plaque and bone formation .
	manualset3
137709	1	407132	5	NULL	NULL	0	NULL	Six of 52 patients 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six of 52 patients in the cefoxitin group ( 11.5 per cent ) and six of 48 patients in the metronidazole/gentamicin group ( 12.5 per cent ) developed serious wound infections .
	manualset3
137710	2	407132	5	NULL	NULL	0	NULL	cefoxitin group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Six of 52 patients in the cefoxitin group ( 11.5 per cent ) and six of 48 patients in the metronidazole/gentamicin group ( 12.5 per cent ) developed serious wound infections .
	manualset3
137711	3	407132	5	NULL	NULL	0	NULL	11.5 per cent	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six of 52 patients in the cefoxitin group ( 11.5 per cent ) and six of 48 patients in the metronidazole/gentamicin group ( 12.5 per cent ) developed serious wound infections .
	manualset3
137712	4	407132	5	NULL	NULL	0	NULL	six of 48 patients 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six of 52 patients in the cefoxitin group ( 11.5 per cent ) and six of 48 patients in the metronidazole/gentamicin group ( 12.5 per cent ) developed serious wound infections .
	manualset3
137713	5	407132	5	NULL	NULL	0	NULL	metronidazole/gentamicin group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Six of 52 patients in the cefoxitin group ( 11.5 per cent ) and six of 48 patients in the metronidazole/gentamicin group ( 12.5 per cent ) developed serious wound infections .
	manualset3
137714	6	407132	5	NULL	NULL	0	NULL	12.5 per cent 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six of 52 patients in the cefoxitin group ( 11.5 per cent ) and six of 48 patients in the metronidazole/gentamicin group ( 12.5 per cent ) developed serious wound infections .
	manualset3
137715	7	407132	5	NULL	NULL	0	NULL	serious wound infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Six of 52 patients in the cefoxitin group ( 11.5 per cent ) and six of 48 patients in the metronidazole/gentamicin group ( 12.5 per cent ) developed serious wound infections .
	manualset3
137716	1	407133	5	NULL	NULL	0	NULL	Six of the 36 carcinomas	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six of the 36 carcinomas were positive for EGFR .
	manualset3
137717	2	407133	5	NULL	NULL	0	NULL	EGFR 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Six of the 36 carcinomas were positive for EGFR .
	manualset3
137718	1	407134	5	NULL	NULL	0	NULL	Six 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six optimized neural networks were produced to investigate the impact of different input information on WMC segmentation .
	manualset3
137719	2	407134	5	NULL	NULL	0	NULL	neural networks	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Six optimized neural networks were produced to investigate the impact of different input information on WMC segmentation .
	manualset3
137720	3	407134	5	NULL	NULL	0	NULL	impact 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Six optimized neural networks were produced to investigate the impact of different input information on WMC segmentation .
	manualset3
137721	4	407134	5	NULL	NULL	0	NULL	different input information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Six optimized neural networks were produced to investigate the impact of different input information on WMC segmentation .
	manualset3
137722	5	407134	5	NULL	NULL	0	NULL	WMC segmentation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Six optimized neural networks were produced to investigate the impact of different input information on WMC segmentation .
	manualset3
137723	1	407135	5	NULL	NULL	0	NULL	Six or seven 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six or seven high abundance glycoproteins were identified for EHV-4 , EHV-1 and AHV-3 .
	manualset3
137724	2	407135	5	NULL	NULL	0	NULL	high abundance glycoproteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Six or seven high abundance glycoproteins were identified for EHV-4 , EHV-1 and AHV-3 .
	manualset3
137725	3	407135	5	NULL	NULL	0	NULL	EHV-4	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Six or seven high abundance glycoproteins were identified for EHV-4 , EHV-1 and AHV-3 .
	manualset3
137726	4	407135	5	NULL	NULL	0	NULL	EHV-1	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Six or seven high abundance glycoproteins were identified for EHV-4 , EHV-1 and AHV-3 .
	manualset3
137727	5	407135	5	NULL	NULL	0	NULL	AHV-3 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Six or seven high abundance glycoproteins were identified for EHV-4 , EHV-1 and AHV-3 .
	manualset3
137728	1	407136	5	NULL	NULL	0	NULL	Six patients	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six patients underwent surgical exploration ; removal of the lesions halted the progression of symptoms in five patients , and one patient had worsened sensory function after surgery .
	manualset3
137729	2	407136	5	NULL	NULL	0	NULL	surgical exploration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Six patients underwent surgical exploration ; removal of the lesions halted the progression of symptoms in five patients , and one patient had worsened sensory function after surgery .
	manualset3
137730	3	407136	5	NULL	NULL	0	NULL	removal 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Six patients underwent surgical exploration ; removal of the lesions halted the progression of symptoms in five patients , and one patient had worsened sensory function after surgery .
	manualset3
137731	4	407136	5	NULL	NULL	0	NULL	lesions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Six patients underwent surgical exploration ; removal of the lesions halted the progression of symptoms in five patients , and one patient had worsened sensory function after surgery .
	manualset3
137732	5	407136	5	NULL	NULL	0	NULL	progression 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Six patients underwent surgical exploration ; removal of the lesions halted the progression of symptoms in five patients , and one patient had worsened sensory function after surgery .
	manualset3
137733	6	407136	5	NULL	NULL	0	NULL	symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Six patients underwent surgical exploration ; removal of the lesions halted the progression of symptoms in five patients , and one patient had worsened sensory function after surgery .
	manualset3
137734	7	407136	5	NULL	NULL	0	NULL	five patients 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six patients underwent surgical exploration ; removal of the lesions halted the progression of symptoms in five patients , and one patient had worsened sensory function after surgery .
	manualset3
137735	8	407136	5	NULL	NULL	0	NULL	one patient	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six patients underwent surgical exploration ; removal of the lesions halted the progression of symptoms in five patients , and one patient had worsened sensory function after surgery .
	manualset3
137736	9	407136	5	NULL	NULL	0	NULL	worsened sensory function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Six patients underwent surgical exploration ; removal of the lesions halted the progression of symptoms in five patients , and one patient had worsened sensory function after surgery .
	manualset3
137737	10	407136	5	NULL	NULL	0	NULL	surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Six patients underwent surgical exploration ; removal of the lesions halted the progression of symptoms in five patients , and one patient had worsened sensory function after surgery .
	manualset3
137738	1	407137	5	NULL	NULL	0	NULL	Six primary tumors 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six primary tumors , diagnosed by increased calcitonin levels , were all correctly diagnosed ; 47 recurrences , also suspected by blood tumor markers , were detected and confirmed by cytology or histology .
	manualset3
137739	2	407137	5	NULL	NULL	0	NULL	calcitonin levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Six primary tumors , diagnosed by increased calcitonin levels , were all correctly diagnosed ; 47 recurrences , also suspected by blood tumor markers , were detected and confirmed by cytology or histology .
	manualset3
137740	3	407137	5	NULL	NULL	0	NULL	47 recurrences 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six primary tumors , diagnosed by increased calcitonin levels , were all correctly diagnosed ; 47 recurrences , also suspected by blood tumor markers , were detected and confirmed by cytology or histology .
	manualset3
137741	4	407137	5	NULL	NULL	0	NULL	blood tumor markers 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Six primary tumors , diagnosed by increased calcitonin levels , were all correctly diagnosed ; 47 recurrences , also suspected by blood tumor markers , were detected and confirmed by cytology or histology .
	manualset3
137742	5	407137	5	NULL	NULL	0	NULL	cytology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Six primary tumors , diagnosed by increased calcitonin levels , were all correctly diagnosed ; 47 recurrences , also suspected by blood tumor markers , were detected and confirmed by cytology or histology .
	manualset3
137743	6	407137	5	NULL	NULL	0	NULL	histology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Six primary tumors , diagnosed by increased calcitonin levels , were all correctly diagnosed ; 47 recurrences , also suspected by blood tumor markers , were detected and confirmed by cytology or histology .
	manualset3
137744	1	407138	5	NULL	NULL	0	NULL	Six putative lignin peroxidase ( LIP ) genes	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six putative lignin peroxidase ( LIP ) genes were isolated from a lambda EMBL3 phage library of the white-rot fungus , Trametes versicolor , using the Phanerochaete chrysosporium LIP cDNA CLG5 as the probe .
	manualset3
137745	2	407138	5	NULL	NULL	0	NULL	lambda EMBL3 phage library	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Six putative lignin peroxidase ( LIP ) genes were isolated from a lambda EMBL3 phage library of the white-rot fungus , Trametes versicolor , using the Phanerochaete chrysosporium LIP cDNA CLG5 as the probe .
	manualset3
137746	3	407138	5	NULL	NULL	0	NULL	white-rot fungus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Six putative lignin peroxidase ( LIP ) genes were isolated from a lambda EMBL3 phage library of the white-rot fungus , Trametes versicolor , using the Phanerochaete chrysosporium LIP cDNA CLG5 as the probe .
	manualset3
137747	4	407138	5	NULL	NULL	0	NULL	Trametes versicolor	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Six putative lignin peroxidase ( LIP ) genes were isolated from a lambda EMBL3 phage library of the white-rot fungus , Trametes versicolor , using the Phanerochaete chrysosporium LIP cDNA CLG5 as the probe .
	manualset3
137748	5	407138	5	NULL	NULL	0	NULL	Phanerochaete chrysosporium LIP cDNA CLG5	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Six putative lignin peroxidase ( LIP ) genes were isolated from a lambda EMBL3 phage library of the white-rot fungus , Trametes versicolor , using the Phanerochaete chrysosporium LIP cDNA CLG5 as the probe .
	manualset3
137749	6	407138	5	NULL	NULL	0	NULL	probe 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Six putative lignin peroxidase ( LIP ) genes were isolated from a lambda EMBL3 phage library of the white-rot fungus , Trametes versicolor , using the Phanerochaete chrysosporium LIP cDNA CLG5 as the probe .
	manualset3
137750	1	407139	5	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of studies suggest that there is a genetic basis for the formation by some hemophilia A patients of antibodies that inactivate factor VIII .
	manualset3
137751	2	407139	5	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of studies suggest that there is a genetic basis for the formation by some hemophilia A patients of antibodies that inactivate factor VIII .
	manualset3
137752	3	407139	5	NULL	NULL	0	NULL	genetic basis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of studies suggest that there is a genetic basis for the formation by some hemophilia A patients of antibodies that inactivate factor VIII .
	manualset3
137753	4	407139	5	NULL	NULL	0	NULL	formation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of studies suggest that there is a genetic basis for the formation by some hemophilia A patients of antibodies that inactivate factor VIII .
	manualset3
137754	5	407139	5	NULL	NULL	0	NULL	hemophilia A patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of studies suggest that there is a genetic basis for the formation by some hemophilia A patients of antibodies that inactivate factor VIII .
	manualset3
137755	6	407139	5	NULL	NULL	0	NULL	antibodies 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of studies suggest that there is a genetic basis for the formation by some hemophilia A patients of antibodies that inactivate factor VIII .
	manualset3
137756	7	407139	5	NULL	NULL	0	NULL	factor VIII	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of studies suggest that there is a genetic basis for the formation by some hemophilia A patients of antibodies that inactivate factor VIII .
	manualset3
137757	1	407140	5	NULL	NULL	0	NULL	Six themes	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six themes were identified : ( 1 ) screening and referral , ( 2 ) facilitators to referral , ( 3 ) barriers to referral , ( 4 ) culture and language , ( 5 ) life events , and ( 6 ) support .
	manualset3
137758	2	407140	5	NULL	NULL	0	NULL	screening 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Six themes were identified : ( 1 ) screening and referral , ( 2 ) facilitators to referral , ( 3 ) barriers to referral , ( 4 ) culture and language , ( 5 ) life events , and ( 6 ) support .
	manualset3
137759	3	407140	5	NULL	NULL	0	NULL	referral 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Six themes were identified : ( 1 ) screening and referral , ( 2 ) facilitators to referral , ( 3 ) barriers to referral , ( 4 ) culture and language , ( 5 ) life events , and ( 6 ) support .
	manualset3
137760	4	407140	5	NULL	NULL	0	NULL	facilitators 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Six themes were identified : ( 1 ) screening and referral , ( 2 ) facilitators to referral , ( 3 ) barriers to referral , ( 4 ) culture and language , ( 5 ) life events , and ( 6 ) support .
	manualset3
137761	5	407140	5	NULL	NULL	0	NULL	referral 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Six themes were identified : ( 1 ) screening and referral , ( 2 ) facilitators to referral , ( 3 ) barriers to referral , ( 4 ) culture and language , ( 5 ) life events , and ( 6 ) support .
	manualset3
137762	6	407140	5	NULL	NULL	0	NULL	barriers 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Six themes were identified : ( 1 ) screening and referral , ( 2 ) facilitators to referral , ( 3 ) barriers to referral , ( 4 ) culture and language , ( 5 ) life events , and ( 6 ) support .
	manualset3
137763	7	407140	5	NULL	NULL	0	NULL	referral 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Six themes were identified : ( 1 ) screening and referral , ( 2 ) facilitators to referral , ( 3 ) barriers to referral , ( 4 ) culture and language , ( 5 ) life events , and ( 6 ) support .
	manualset3
137764	8	407140	5	NULL	NULL	0	NULL	culture 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Six themes were identified : ( 1 ) screening and referral , ( 2 ) facilitators to referral , ( 3 ) barriers to referral , ( 4 ) culture and language , ( 5 ) life events , and ( 6 ) support .
	manualset3
137765	9	407140	5	NULL	NULL	0	NULL	language 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Six themes were identified : ( 1 ) screening and referral , ( 2 ) facilitators to referral , ( 3 ) barriers to referral , ( 4 ) culture and language , ( 5 ) life events , and ( 6 ) support .
	manualset3
137766	10	407140	5	NULL	NULL	0	NULL	life events	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Six themes were identified : ( 1 ) screening and referral , ( 2 ) facilitators to referral , ( 3 ) barriers to referral , ( 4 ) culture and language , ( 5 ) life events , and ( 6 ) support .
	manualset3
137767	11	407140	5	NULL	NULL	0	NULL	support 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Six themes were identified : ( 1 ) screening and referral , ( 2 ) facilitators to referral , ( 3 ) barriers to referral , ( 4 ) culture and language , ( 5 ) life events , and ( 6 ) support .
	manualset3
137768	1	407141	5	NULL	NULL	0	NULL	Six triterpenoid saponins 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Six triterpenoid saponins were isolated from the edible grain quinoa , which is seeds of Chenopodium quinoa ( Chenopodiaceae ) .
	manualset3
137769	2	407141	5	NULL	NULL	NULL	NULL	edible grain quinoa	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Six triterpenoid saponins were isolated from the edible grain quinoa , which is seeds of Chenopodium quinoa ( Chenopodiaceae ) .
	manualset3
137770	3	407141	5	NULL	NULL	0	NULL	seeds 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Six triterpenoid saponins were isolated from the edible grain quinoa , which is seeds of Chenopodium quinoa ( Chenopodiaceae ) .
	manualset3
137771	4	407141	5	NULL	NULL	0	NULL	Chenopodium quinoa ( Chenopodiaceae ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Six triterpenoid saponins were isolated from the edible grain quinoa , which is seeds of Chenopodium quinoa ( Chenopodiaceae ) .
	manualset3
137772	1	407142	5	NULL	NULL	0	NULL	Sixteen 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixteen healthy men were evaluated for left ventricular performance changes and beta-blockade after therapeutic oral doses of disopyramide and propranolol administered alone and concurrently .
	manualset3
137773	2	407142	5	NULL	NULL	0	NULL	healthy men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixteen healthy men were evaluated for left ventricular performance changes and beta-blockade after therapeutic oral doses of disopyramide and propranolol administered alone and concurrently .
	manualset3
137774	3	407142	5	NULL	NULL	0	NULL	left ventricular performance changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixteen healthy men were evaluated for left ventricular performance changes and beta-blockade after therapeutic oral doses of disopyramide and propranolol administered alone and concurrently .
	manualset3
137775	4	407142	5	NULL	NULL	0	NULL	beta-blockade	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixteen healthy men were evaluated for left ventricular performance changes and beta-blockade after therapeutic oral doses of disopyramide and propranolol administered alone and concurrently .
	manualset3
137776	5	407142	5	NULL	NULL	0	NULL	therapeutic oral doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixteen healthy men were evaluated for left ventricular performance changes and beta-blockade after therapeutic oral doses of disopyramide and propranolol administered alone and concurrently .
	manualset3
137777	6	407142	5	NULL	NULL	0	NULL	disopyramide 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixteen healthy men were evaluated for left ventricular performance changes and beta-blockade after therapeutic oral doses of disopyramide and propranolol administered alone and concurrently .
	manualset3
137778	7	407142	5	NULL	NULL	0	NULL	propranolol 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixteen healthy men were evaluated for left ventricular performance changes and beta-blockade after therapeutic oral doses of disopyramide and propranolol administered alone and concurrently .
	manualset3
137779	1	407143	5	NULL	NULL	0	NULL	Sixteen 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixteen ovariectomized hinds received a protocol of steroid treatment to mimic ovarian hormone secretion during the normal oestrous cycle .
	manualset3
137780	2	407143	5	NULL	NULL	0	NULL	ovariectomized hinds	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixteen ovariectomized hinds received a protocol of steroid treatment to mimic ovarian hormone secretion during the normal oestrous cycle .
	manualset3
137781	3	407143	5	NULL	NULL	0	NULL	protocol 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixteen ovariectomized hinds received a protocol of steroid treatment to mimic ovarian hormone secretion during the normal oestrous cycle .
	manualset3
137782	4	407143	5	NULL	NULL	0	NULL	steroid treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixteen ovariectomized hinds received a protocol of steroid treatment to mimic ovarian hormone secretion during the normal oestrous cycle .
	manualset3
137783	5	407143	5	NULL	NULL	0	NULL	ovarian hormone secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixteen ovariectomized hinds received a protocol of steroid treatment to mimic ovarian hormone secretion during the normal oestrous cycle .
	manualset3
137784	6	407143	5	NULL	NULL	0	NULL	normal oestrous cycle	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixteen ovariectomized hinds received a protocol of steroid treatment to mimic ovarian hormone secretion during the normal oestrous cycle .
	manualset3
137785	1	407144	5	NULL	NULL	0	NULL	Sixteen 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixteen pyridonecarboxylic acids , characterized by having a chlorine atom and a cyclopropyl group at the 6 - and 1-position respectively , substituted amino groups at the 7-position , and some substituted groups ( chloro , nitro , amino , dimethylamino ) at the 8-position , were synthesized .
	manualset3
137786	2	407144	5	NULL	NULL	0	NULL	pyridonecarboxylic acids	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixteen pyridonecarboxylic acids , characterized by having a chlorine atom and a cyclopropyl group at the 6 - and 1-position respectively , substituted amino groups at the 7-position , and some substituted groups ( chloro , nitro , amino , dimethylamino ) at the 8-position , were synthesized .
	manualset3
137787	3	407144	5	NULL	NULL	0	NULL	chlorine atom	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixteen pyridonecarboxylic acids , characterized by having a chlorine atom and a cyclopropyl group at the 6 - and 1-position respectively , substituted amino groups at the 7-position , and some substituted groups ( chloro , nitro , amino , dimethylamino ) at the 8-position , were synthesized .
	manualset3
137788	4	407144	5	NULL	NULL	0	NULL	cyclopropyl group	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixteen pyridonecarboxylic acids , characterized by having a chlorine atom and a cyclopropyl group at the 6 - and 1-position respectively , substituted amino groups at the 7-position , and some substituted groups ( chloro , nitro , amino , dimethylamino ) at the 8-position , were synthesized .
	manualset3
137789	5	407144	5	NULL	NULL	0	NULL	 6 -position	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixteen pyridonecarboxylic acids , characterized by having a chlorine atom and a cyclopropyl group at the 6 - and 1-position respectively , substituted amino groups at the 7-position , and some substituted groups ( chloro , nitro , amino , dimethylamino ) at the 8-position , were synthesized .
	manualset3
137790	6	407144	5	NULL	NULL	0	NULL	1-position	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixteen pyridonecarboxylic acids , characterized by having a chlorine atom and a cyclopropyl group at the 6 - and 1-position respectively , substituted amino groups at the 7-position , and some substituted groups ( chloro , nitro , amino , dimethylamino ) at the 8-position , were synthesized .
	manualset3
137791	7	407144	5	NULL	NULL	0	NULL	substituted amino groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixteen pyridonecarboxylic acids , characterized by having a chlorine atom and a cyclopropyl group at the 6 - and 1-position respectively , substituted amino groups at the 7-position , and some substituted groups ( chloro , nitro , amino , dimethylamino ) at the 8-position , were synthesized .
	manualset3
137792	8	407144	5	NULL	NULL	0	NULL	7-position	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixteen pyridonecarboxylic acids , characterized by having a chlorine atom and a cyclopropyl group at the 6 - and 1-position respectively , substituted amino groups at the 7-position , and some substituted groups ( chloro , nitro , amino , dimethylamino ) at the 8-position , were synthesized .
	manualset3
137793	9	407144	5	NULL	NULL	0	NULL	substituted groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixteen pyridonecarboxylic acids , characterized by having a chlorine atom and a cyclopropyl group at the 6 - and 1-position respectively , substituted amino groups at the 7-position , and some substituted groups ( chloro , nitro , amino , dimethylamino ) at the 8-position , were synthesized .
	manualset3
137794	10	407144	5	NULL	NULL	0	NULL	chloro 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixteen pyridonecarboxylic acids , characterized by having a chlorine atom and a cyclopropyl group at the 6 - and 1-position respectively , substituted amino groups at the 7-position , and some substituted groups ( chloro , nitro , amino , dimethylamino ) at the 8-position , were synthesized .
	manualset3
137795	11	407144	5	NULL	NULL	0	NULL	nitro 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixteen pyridonecarboxylic acids , characterized by having a chlorine atom and a cyclopropyl group at the 6 - and 1-position respectively , substituted amino groups at the 7-position , and some substituted groups ( chloro , nitro , amino , dimethylamino ) at the 8-position , were synthesized .
	manualset3
137796	12	407144	5	NULL	NULL	0	NULL	amino 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixteen pyridonecarboxylic acids , characterized by having a chlorine atom and a cyclopropyl group at the 6 - and 1-position respectively , substituted amino groups at the 7-position , and some substituted groups ( chloro , nitro , amino , dimethylamino ) at the 8-position , were synthesized .
	manualset3
137797	13	407144	5	NULL	NULL	0	NULL	dimethylamino 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixteen pyridonecarboxylic acids , characterized by having a chlorine atom and a cyclopropyl group at the 6 - and 1-position respectively , substituted amino groups at the 7-position , and some substituted groups ( chloro , nitro , amino , dimethylamino ) at the 8-position , were synthesized .
	manualset3
137798	14	407144	5	NULL	NULL	0	NULL	8-position	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixteen pyridonecarboxylic acids , characterized by having a chlorine atom and a cyclopropyl group at the 6 - and 1-position respectively , substituted amino groups at the 7-position , and some substituted groups ( chloro , nitro , amino , dimethylamino ) at the 8-position , were synthesized .
	manualset3
137799	1	407145	5	NULL	NULL	0	NULL	Sixty-four 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty-four Sprague-Dawley rats underwent an 80 % small bowel resection or transection as control .
	manualset3
137800	2	407145	5	NULL	NULL	0	NULL	Sprague-Dawley rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty-four Sprague-Dawley rats underwent an 80 % small bowel resection or transection as control .
	manualset3
137801	3	407145	5	NULL	NULL	0	NULL	80 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty-four Sprague-Dawley rats underwent an 80 % small bowel resection or transection as control .
	manualset3
137802	4	407145	5	NULL	NULL	0	NULL	small bowel resection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty-four Sprague-Dawley rats underwent an 80 % small bowel resection or transection as control .
	manualset3
137803	5	407145	5	NULL	NULL	0	NULL	transection 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty-four Sprague-Dawley rats underwent an 80 % small bowel resection or transection as control .
	manualset3
137804	6	407145	5	NULL	NULL	0	NULL	control 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty-four Sprague-Dawley rats underwent an 80 % small bowel resection or transection as control .
	manualset3
137805	1	407146	5	NULL	NULL	0	NULL	Sixty-one per cent 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty-one per cent of these patients had Stage I disease , 21 % Stage II disease , 16 % Stage III and 2 % Stage IV .
	manualset3
137806	2	407146	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty-one per cent of these patients had Stage I disease , 21 % Stage II disease , 16 % Stage III and 2 % Stage IV .
	manualset3
137807	3	407146	5	NULL	NULL	NULL	NULL	Stage I disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Sixty-one per cent of these patients had Stage I disease , 21 % Stage II disease , 16 % Stage III and 2 % Stage IV .
	manualset3
137808	4	407146	5	NULL	NULL	0	NULL	21 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty-one per cent of these patients had Stage I disease , 21 % Stage II disease , 16 % Stage III and 2 % Stage IV .
	manualset3
137809	5	407146	5	NULL	NULL	NULL	NULL	Stage II disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Sixty-one per cent of these patients had Stage I disease , 21 % Stage II disease , 16 % Stage III and 2 % Stage IV .
	manualset3
137810	6	407146	5	NULL	NULL	0	NULL	16 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty-one per cent of these patients had Stage I disease , 21 % Stage II disease , 16 % Stage III and 2 % Stage IV .
	manualset3
137811	7	407146	5	NULL	NULL	NULL	NULL	Stage III 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Sixty-one per cent of these patients had Stage I disease , 21 % Stage II disease , 16 % Stage III and 2 % Stage IV .
	manualset3
137812	8	407146	5	NULL	NULL	0	NULL	2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty-one per cent of these patients had Stage I disease , 21 % Stage II disease , 16 % Stage III and 2 % Stage IV .
	manualset3
137813	9	407146	5	NULL	NULL	NULL	NULL	Stage IV	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Sixty-one per cent of these patients had Stage I disease , 21 % Stage II disease , 16 % Stage III and 2 % Stage IV .
	manualset3
137814	1	407147	5	NULL	NULL	0	NULL	Sixty-two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty-two intervention studies reported mixed results , which did not depend on sample size or duration of the intervention .
	manualset3
137815	2	407147	5	NULL	NULL	0	NULL	intervention studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty-two intervention studies reported mixed results , which did not depend on sample size or duration of the intervention .
	manualset3
137816	3	407147	5	NULL	NULL	0	NULL	mixed results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty-two intervention studies reported mixed results , which did not depend on sample size or duration of the intervention .
	manualset3
137817	4	407147	5	NULL	NULL	0	NULL	sample size	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty-two intervention studies reported mixed results , which did not depend on sample size or duration of the intervention .
	manualset3
137818	5	407147	5	NULL	NULL	0	NULL	duration 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty-two intervention studies reported mixed results , which did not depend on sample size or duration of the intervention .
	manualset3
137819	6	407147	5	NULL	NULL	0	NULL	intervention 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty-two intervention studies reported mixed results , which did not depend on sample size or duration of the intervention .
	manualset3
137820	1	407148	5	NULL	NULL	0	NULL	Sixty-two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty-two patients with vertigo were examined with ABR .
	manualset3
137821	2	407148	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty-two patients with vertigo were examined with ABR .
	manualset3
137822	3	407148	5	NULL	NULL	0	NULL	vertigo 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty-two patients with vertigo were examined with ABR .
	manualset3
137823	4	407148	5	NULL	NULL	0	NULL	ABR 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty-two patients with vertigo were examined with ABR .
	manualset3
137824	1	407149	5	NULL	NULL	0	NULL	Size-exclusion high-performance liquid chromatography ( SE-HPLC , SEC ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Size-exclusion high-performance liquid chromatography ( SE-HPLC , SEC ) is the long-standing biopharmaceutical industry standard for quantitation of soluble protein aggregates .
	manualset3
137825	2	407149	5	NULL	NULL	0	NULL	biopharmaceutical industry standard	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Size-exclusion high-performance liquid chromatography ( SE-HPLC , SEC ) is the long-standing biopharmaceutical industry standard for quantitation of soluble protein aggregates .
	manualset3
137826	3	407149	5	NULL	NULL	0	NULL	quantitation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Size-exclusion high-performance liquid chromatography ( SE-HPLC , SEC ) is the long-standing biopharmaceutical industry standard for quantitation of soluble protein aggregates .
	manualset3
137827	4	407149	5	NULL	NULL	0	NULL	soluble protein aggregates	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Size-exclusion high-performance liquid chromatography ( SE-HPLC , SEC ) is the long-standing biopharmaceutical industry standard for quantitation of soluble protein aggregates .
	manualset3
137828	1	407150	5	NULL	NULL	0	NULL	Skeletal metastases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Skeletal metastases from cancer of the uterine cervix : frequency , patterns , and radiotherapeutic significance .
	manualset3
137829	2	407150	5	NULL	NULL	0	NULL	cancer of the uterine cervix	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Skeletal metastases from cancer of the uterine cervix : frequency , patterns , and radiotherapeutic significance .
	manualset3
137830	3	407150	5	NULL	NULL	0	NULL	frequency 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Skeletal metastases from cancer of the uterine cervix : frequency , patterns , and radiotherapeutic significance .
	manualset3
137831	4	407150	5	NULL	NULL	0	NULL	patterns 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Skeletal metastases from cancer of the uterine cervix : frequency , patterns , and radiotherapeutic significance .
	manualset3
137832	5	407150	5	NULL	NULL	0	NULL	radiotherapeutic significance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Skeletal metastases from cancer of the uterine cervix : frequency , patterns , and radiotherapeutic significance .
	manualset3
137833	1	407151	5	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of subtle changes , however , have been detected in the structure of each derivative compared with that of the native toxin .
	manualset3
137834	2	407151	5	NULL	NULL	0	NULL	subtle changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of subtle changes , however , have been detected in the structure of each derivative compared with that of the native toxin .
	manualset3
137835	3	407151	5	NULL	NULL	0	NULL	structure 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of subtle changes , however , have been detected in the structure of each derivative compared with that of the native toxin .
	manualset3
137836	4	407151	5	NULL	NULL	0	NULL	derivative 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of subtle changes , however , have been detected in the structure of each derivative compared with that of the native toxin .
	manualset3
137837	5	407151	5	NULL	NULL	0	NULL	native toxin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of subtle changes , however , have been detected in the structure of each derivative compared with that of the native toxin .
	manualset3
137838	1	407152	5	NULL	NULL	0	NULL	Skeletal muscle	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Skeletal muscle as a myocardial substitute .
	manualset3
137839	2	407152	5	NULL	NULL	0	NULL	myocardial substitute	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Skeletal muscle as a myocardial substitute .
	manualset3
137840	1	407153	5	NULL	NULL	0	NULL	Ski/Sno	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Ski/Sno also suppress transcription induced by multiple activators , such as Smads and c-Myb .
	manualset3
137841	2	407153	5	NULL	NULL	0	NULL	transcription 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ski/Sno also suppress transcription induced by multiple activators , such as Smads and c-Myb .
	manualset3
137842	3	407153	5	NULL	NULL	0	NULL	multiple activators	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ski/Sno also suppress transcription induced by multiple activators , such as Smads and c-Myb .
	manualset3
137843	4	407153	5	NULL	NULL	0	NULL	Smads 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ski/Sno also suppress transcription induced by multiple activators , such as Smads and c-Myb .
	manualset3
137844	5	407153	5	NULL	NULL	0	NULL	c-Myb 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Ski/Sno also suppress transcription induced by multiple activators , such as Smads and c-Myb .
	manualset3
137845	1	407154	5	NULL	NULL	0	NULL	Skin biopsy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin biopsy was compatible with verrucous epidermal nevus while the biopsy of the ocular lesion confirmed complex choristoma .
	manualset3
137846	2	407154	5	NULL	NULL	0	NULL	verrucous epidermal nevus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin biopsy was compatible with verrucous epidermal nevus while the biopsy of the ocular lesion confirmed complex choristoma .
	manualset3
137847	3	407154	5	NULL	NULL	0	NULL	biopsy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin biopsy was compatible with verrucous epidermal nevus while the biopsy of the ocular lesion confirmed complex choristoma .
	manualset3
137848	4	407154	5	NULL	NULL	0	NULL	ocular lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin biopsy was compatible with verrucous epidermal nevus while the biopsy of the ocular lesion confirmed complex choristoma .
	manualset3
137849	5	407154	5	NULL	NULL	0	NULL	complex choristoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin biopsy was compatible with verrucous epidermal nevus while the biopsy of the ocular lesion confirmed complex choristoma .
	manualset3
137850	1	407155	5	NULL	NULL	0	NULL	Skin cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin cancer after nonmyeloablative hematopoietic cell transplantation .
	manualset3
137851	2	407155	5	NULL	NULL	0	NULL	nonmyeloablative hematopoietic cell transplantation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin cancer after nonmyeloablative hematopoietic cell transplantation .
	manualset3
137852	1	407156	5	NULL	NULL	0	NULL	Skin cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin cancer is the most common cancer in humans .
	manualset3
137853	2	407156	5	NULL	NULL	0	NULL	common cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin cancer is the most common cancer in humans .
	manualset3
137854	3	407156	5	NULL	NULL	0	NULL	humans 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin cancer is the most common cancer in humans .
	manualset3
137855	1	407157	5	NULL	NULL	0	NULL	Skin cell-mediated BMP2 therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin cell-mediated BMP2 therapy may be considered as a potential treatment for various types of fractures and bone defects .
	manualset3
137856	2	407157	5	NULL	NULL	0	NULL	potential treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin cell-mediated BMP2 therapy may be considered as a potential treatment for various types of fractures and bone defects .
	manualset3
137857	3	407157	5	NULL	NULL	0	NULL	various types of fractures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin cell-mediated BMP2 therapy may be considered as a potential treatment for various types of fractures and bone defects .
	manualset3
137858	4	407157	5	NULL	NULL	0	NULL	bone defects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin cell-mediated BMP2 therapy may be considered as a potential treatment for various types of fractures and bone defects .
	manualset3
137859	1	407158	5	NULL	NULL	0	NULL	Skin hyperirritability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin hyperirritability to irritants as well as atopy are considered to be predisposing factors for contact dermatitis .
	manualset3
137860	2	407158	5	NULL	NULL	0	NULL	irritants 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin hyperirritability to irritants as well as atopy are considered to be predisposing factors for contact dermatitis .
	manualset3
137861	3	407158	5	NULL	NULL	0	NULL	atopy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin hyperirritability to irritants as well as atopy are considered to be predisposing factors for contact dermatitis .
	manualset3
137862	4	407158	5	NULL	NULL	0	NULL	predisposing factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin hyperirritability to irritants as well as atopy are considered to be predisposing factors for contact dermatitis .
	manualset3
137863	5	407158	5	NULL	NULL	0	NULL	contact dermatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin hyperirritability to irritants as well as atopy are considered to be predisposing factors for contact dermatitis .
	manualset3
137864	1	407159	5	NULL	NULL	0	NULL	Skin inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin inflammation in atopic dermatitis ( AD ) is characterized by the predominant infiltration of T-helper ( Th ) 2-cells in lesional skin .
	manualset3
137865	2	407159	5	NULL	NULL	0	NULL	atopic dermatitis ( AD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin inflammation in atopic dermatitis ( AD ) is characterized by the predominant infiltration of T-helper ( Th ) 2-cells in lesional skin .
	manualset3
137866	3	407159	5	NULL	NULL	0	NULL	predominant infiltration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin inflammation in atopic dermatitis ( AD ) is characterized by the predominant infiltration of T-helper ( Th ) 2-cells in lesional skin .
	manualset3
137867	4	407159	5	NULL	NULL	0	NULL	T-helper ( Th ) 2-cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin inflammation in atopic dermatitis ( AD ) is characterized by the predominant infiltration of T-helper ( Th ) 2-cells in lesional skin .
	manualset3
137868	5	407159	5	NULL	NULL	0	NULL	lesional skin	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin inflammation in atopic dermatitis ( AD ) is characterized by the predominant infiltration of T-helper ( Th ) 2-cells in lesional skin .
	manualset3
137869	1	407160	5	NULL	NULL	0	NULL	Skin metastasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin metastasis is rare in teratocarcinoma of the testis ( 1 ) .
	manualset3
137870	2	407160	5	NULL	NULL	0	NULL	teratocarcinoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin metastasis is rare in teratocarcinoma of the testis ( 1 ) .
	manualset3
137871	3	407160	5	NULL	NULL	0	NULL	testis 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin metastasis is rare in teratocarcinoma of the testis ( 1 ) .
	manualset3
137872	1	407161	5	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of suggestions for human and animal researchers are made in order to address these phenotypes and enhance consilience .
	manualset3
137873	2	407161	5	NULL	NULL	0	NULL	suggestions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of suggestions for human and animal researchers are made in order to address these phenotypes and enhance consilience .
	manualset3
137874	3	407161	5	NULL	NULL	0	NULL	human researchers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of suggestions for human and animal researchers are made in order to address these phenotypes and enhance consilience .
	manualset3
137875	4	407161	5	NULL	NULL	0	NULL	animal researchers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of suggestions for human and animal researchers are made in order to address these phenotypes and enhance consilience .
	manualset3
137876	5	407161	5	NULL	NULL	0	NULL	phenotypes 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of suggestions for human and animal researchers are made in order to address these phenotypes and enhance consilience .
	manualset3
137877	6	407161	5	NULL	NULL	0	NULL	consilience 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of suggestions for human and animal researchers are made in order to address these phenotypes and enhance consilience .
	manualset3
137878	1	407162	5	NULL	NULL	0	NULL	Skin temperature measurements 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin temperature measurements before and after immersion in cold water ( 5 degrees C , for 10 min ) could not be used for the estimation of VWF severity .
	manualset3
137879	2	407162	5	NULL	NULL	0	NULL	immersion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin temperature measurements before and after immersion in cold water ( 5 degrees C , for 10 min ) could not be used for the estimation of VWF severity .
	manualset3
137880	3	407162	5	NULL	NULL	0	NULL	cold water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin temperature measurements before and after immersion in cold water ( 5 degrees C , for 10 min ) could not be used for the estimation of VWF severity .
	manualset3
137881	4	407162	5	NULL	NULL	0	NULL	5 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin temperature measurements before and after immersion in cold water ( 5 degrees C , for 10 min ) could not be used for the estimation of VWF severity .
	manualset3
137882	5	407162	5	NULL	NULL	0	NULL	10 min	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin temperature measurements before and after immersion in cold water ( 5 degrees C , for 10 min ) could not be used for the estimation of VWF severity .
	manualset3
137883	6	407162	5	NULL	NULL	0	NULL	estimation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin temperature measurements before and after immersion in cold water ( 5 degrees C , for 10 min ) could not be used for the estimation of VWF severity .
	manualset3
137884	7	407162	5	NULL	NULL	0	NULL	VWF severity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin temperature measurements before and after immersion in cold water ( 5 degrees C , for 10 min ) could not be used for the estimation of VWF severity .
	manualset3
137885	1	407163	5	NULL	NULL	0	NULL	Skin tone	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin tone , hostility , and blood pressure in young normotensive African Americans .
	manualset3
137886	2	407163	5	NULL	NULL	0	NULL	hostility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin tone , hostility , and blood pressure in young normotensive African Americans .
	manualset3
137887	3	407163	5	NULL	NULL	0	NULL	blood pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin tone , hostility , and blood pressure in young normotensive African Americans .
	manualset3
137888	4	407163	5	NULL	NULL	0	NULL	young normotensive African Americans	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin tone , hostility , and blood pressure in young normotensive African Americans .
	manualset3
137889	1	407164	5	NULL	NULL	0	NULL	Skin 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin was smeared with glyciphonic ointment containing 30 % of methylphosphonic diglycidyl ether ( Tatkhimfarmpreparaty Company ) in 495 patients with histologically confirmed basalioma and 36 patients with senile keratosis .
	manualset3
137890	2	407164	5	NULL	NULL	0	NULL	glyciphonic ointment 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin was smeared with glyciphonic ointment containing 30 % of methylphosphonic diglycidyl ether ( Tatkhimfarmpreparaty Company ) in 495 patients with histologically confirmed basalioma and 36 patients with senile keratosis .
	manualset3
137891	3	407164	5	NULL	NULL	0	NULL	30 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin was smeared with glyciphonic ointment containing 30 % of methylphosphonic diglycidyl ether ( Tatkhimfarmpreparaty Company ) in 495 patients with histologically confirmed basalioma and 36 patients with senile keratosis .
	manualset3
137892	4	407164	5	NULL	NULL	0	NULL	methylphosphonic diglycidyl ether	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin was smeared with glyciphonic ointment containing 30 % of methylphosphonic diglycidyl ether ( Tatkhimfarmpreparaty Company ) in 495 patients with histologically confirmed basalioma and 36 patients with senile keratosis .
	manualset3
137893	5	407164	5	NULL	NULL	0	NULL	Tatkhimfarmpreparaty Company	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin was smeared with glyciphonic ointment containing 30 % of methylphosphonic diglycidyl ether ( Tatkhimfarmpreparaty Company ) in 495 patients with histologically confirmed basalioma and 36 patients with senile keratosis .
	manualset3
137894	6	407164	5	NULL	NULL	0	NULL	495 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin was smeared with glyciphonic ointment containing 30 % of methylphosphonic diglycidyl ether ( Tatkhimfarmpreparaty Company ) in 495 patients with histologically confirmed basalioma and 36 patients with senile keratosis .
	manualset3
137895	7	407164	5	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Skin was smeared with glyciphonic ointment containing 30 % of methylphosphonic diglycidyl ether ( Tatkhimfarmpreparaty Company ) in 495 patients with histologically confirmed basalioma and 36 patients with senile keratosis .
	manualset3
137896	8	407164	5	NULL	NULL	0	NULL	basalioma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin was smeared with glyciphonic ointment containing 30 % of methylphosphonic diglycidyl ether ( Tatkhimfarmpreparaty Company ) in 495 patients with histologically confirmed basalioma and 36 patients with senile keratosis .
	manualset3
137897	9	407164	5	NULL	NULL	0	NULL	36 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin was smeared with glyciphonic ointment containing 30 % of methylphosphonic diglycidyl ether ( Tatkhimfarmpreparaty Company ) in 495 patients with histologically confirmed basalioma and 36 patients with senile keratosis .
	manualset3
137898	10	407164	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin was smeared with glyciphonic ointment containing 30 % of methylphosphonic diglycidyl ether ( Tatkhimfarmpreparaty Company ) in 495 patients with histologically confirmed basalioma and 36 patients with senile keratosis .
	manualset3
137899	11	407164	5	NULL	NULL	0	NULL	senile keratosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Skin was smeared with glyciphonic ointment containing 30 % of methylphosphonic diglycidyl ether ( Tatkhimfarmpreparaty Company ) in 495 patients with histologically confirmed basalioma and 36 patients with senile keratosis .
	manualset3
137900	1	407165	5	NULL	NULL	0	NULL	Skull base approach 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Skull base approach to glomus jugulare .
	manualset3
138425	2	407165	5	NULL	NULL	0	NULL	glomus jugulare 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Skull base approach to glomus jugulare .
	manualset3
137901	1	407166	5	NULL	NULL	0	NULL	Sle1 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Sle1 corresponds to at least three subloci , Sle1a , Sle1b , and Sle1c , each of which independently causes loss of tolerance to chromatin , but displays a distinctive immune profile .
	manualset3
137902	2	407166	5	NULL	NULL	0	NULL	three subloci	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sle1 corresponds to at least three subloci , Sle1a , Sle1b , and Sle1c , each of which independently causes loss of tolerance to chromatin , but displays a distinctive immune profile .
	manualset3
137903	3	407166	5	NULL	NULL	0	NULL	Sle1a 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Sle1 corresponds to at least three subloci , Sle1a , Sle1b , and Sle1c , each of which independently causes loss of tolerance to chromatin , but displays a distinctive immune profile .
	manualset3
137904	4	407166	5	NULL	NULL	0	NULL	Sle1b 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Sle1 corresponds to at least three subloci , Sle1a , Sle1b , and Sle1c , each of which independently causes loss of tolerance to chromatin , but displays a distinctive immune profile .
	manualset3
137905	5	407166	5	NULL	NULL	0	NULL	Sle1c 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Sle1 corresponds to at least three subloci , Sle1a , Sle1b , and Sle1c , each of which independently causes loss of tolerance to chromatin , but displays a distinctive immune profile .
	manualset3
137906	6	407166	5	NULL	NULL	0	NULL	loss of tolerance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sle1 corresponds to at least three subloci , Sle1a , Sle1b , and Sle1c , each of which independently causes loss of tolerance to chromatin , but displays a distinctive immune profile .
	manualset3
137907	7	407166	5	NULL	NULL	0	NULL	chromatin 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Sle1 corresponds to at least three subloci , Sle1a , Sle1b , and Sle1c , each of which independently causes loss of tolerance to chromatin , but displays a distinctive immune profile .
	manualset3
137908	8	407166	5	NULL	NULL	0	NULL	distinctive immune profile	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Sle1 corresponds to at least three subloci , Sle1a , Sle1b , and Sle1c , each of which independently causes loss of tolerance to chromatin , but displays a distinctive immune profile .
	manualset3
137909	1	407167	5	NULL	NULL	0	NULL	Sleep-related gastroesophageal reflux	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep-related gastroesophageal reflux : evidence is mounting ...
	manualset3
137910	2	407167	5	NULL	NULL	0	NULL	evidence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep-related gastroesophageal reflux : evidence is mounting ...
	manualset3
137911	1	407168	5	NULL	NULL	0	NULL	Sleep bruxism	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep bruxism may lead to a variety of problems , but its pathophysiology has not been completely elucidated .
	manualset3
137912	2	407168	5	NULL	NULL	0	NULL	problems 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep bruxism may lead to a variety of problems , but its pathophysiology has not been completely elucidated .
	manualset3
137913	3	407168	5	NULL	NULL	0	NULL	pathophysiology 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep bruxism may lead to a variety of problems , but its pathophysiology has not been completely elucidated .
	manualset3
137914	1	407169	5	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of thermodynamic properties such as the pressure , density , heat of evaporation and the surface tension were reliably determined as time averages .
	manualset3
137915	2	407169	5	NULL	NULL	0	NULL	thermodynamic properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of thermodynamic properties such as the pressure , density , heat of evaporation and the surface tension were reliably determined as time averages .
	manualset3
137916	3	407169	5	NULL	NULL	0	NULL	pressure 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of thermodynamic properties such as the pressure , density , heat of evaporation and the surface tension were reliably determined as time averages .
	manualset3
137917	4	407169	5	NULL	NULL	0	NULL	density 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of thermodynamic properties such as the pressure , density , heat of evaporation and the surface tension were reliably determined as time averages .
	manualset3
137918	5	407169	5	NULL	NULL	0	NULL	heat of evaporation 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of thermodynamic properties such as the pressure , density , heat of evaporation and the surface tension were reliably determined as time averages .
	manualset3
137919	6	407169	5	NULL	NULL	0	NULL	surface tension	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of thermodynamic properties such as the pressure , density , heat of evaporation and the surface tension were reliably determined as time averages .
	manualset3
137920	7	407169	5	NULL	NULL	0	NULL	time averages	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of thermodynamic properties such as the pressure , density , heat of evaporation and the surface tension were reliably determined as time averages .
	manualset3
137921	1	407170	5	NULL	NULL	0	NULL	Sleep deprivation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep deprivation ( 24 h ) failed to cause a significant change in any pulmonary function variable ( when controlled for circadian phase ) .
	manualset3
137922	2	407170	5	NULL	NULL	0	NULL	24 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep deprivation ( 24 h ) failed to cause a significant change in any pulmonary function variable ( when controlled for circadian phase ) .
	manualset3
137923	3	407170	5	NULL	NULL	0	NULL	significant change	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep deprivation ( 24 h ) failed to cause a significant change in any pulmonary function variable ( when controlled for circadian phase ) .
	manualset3
137924	4	407170	5	NULL	NULL	0	NULL	pulmonary function variable	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep deprivation ( 24 h ) failed to cause a significant change in any pulmonary function variable ( when controlled for circadian phase ) .
	manualset3
137925	5	407170	5	NULL	NULL	0	NULL	circadian phase	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep deprivation ( 24 h ) failed to cause a significant change in any pulmonary function variable ( when controlled for circadian phase ) .
	manualset3
137926	1	407171	5	NULL	NULL	0	NULL	Sleep problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep problems and their relation to cognitive factors , anxiety , and depressive symptoms in children and adolescents .
	manualset3
137927	2	407171	5	NULL	NULL	0	NULL	relation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep problems and their relation to cognitive factors , anxiety , and depressive symptoms in children and adolescents .
	manualset3
137928	3	407171	5	NULL	NULL	0	NULL	cognitive factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep problems and their relation to cognitive factors , anxiety , and depressive symptoms in children and adolescents .
	manualset3
137929	4	407171	5	NULL	NULL	0	NULL	anxiety 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep problems and their relation to cognitive factors , anxiety , and depressive symptoms in children and adolescents .
	manualset3
137930	5	407171	5	NULL	NULL	0	NULL	depressive symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep problems and their relation to cognitive factors , anxiety , and depressive symptoms in children and adolescents .
	manualset3
137931	6	407171	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep problems and their relation to cognitive factors , anxiety , and depressive symptoms in children and adolescents .
	manualset3
137932	7	407171	5	NULL	NULL	0	NULL	adolescents 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep problems and their relation to cognitive factors , anxiety , and depressive symptoms in children and adolescents .
	manualset3
137933	1	407172	5	NULL	NULL	0	NULL	Sleep studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep studies reveal many patients to have specific sleep abnormalities different from what might be suspected from the clinical history .
	manualset3
137934	2	407172	5	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Sleep studies reveal many patients to have specific sleep abnormalities different from what might be suspected from the clinical history .
	manualset3
137935	3	407172	5	NULL	NULL	0	NULL	specific sleep abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep studies reveal many patients to have specific sleep abnormalities different from what might be suspected from the clinical history .
	manualset3
137936	4	407172	5	NULL	NULL	0	NULL	clinical history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep studies reveal many patients to have specific sleep abnormalities different from what might be suspected from the clinical history .
	manualset3
137937	1	407173	5	NULL	NULL	0	NULL	Sleep studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep studies were performed in seven polio survivors to document objectively abnormal movements in sleep .
	manualset3
137938	2	407173	5	NULL	NULL	0	NULL	seven 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep studies were performed in seven polio survivors to document objectively abnormal movements in sleep .
	manualset3
137939	3	407173	5	NULL	NULL	0	NULL	polio survivors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep studies were performed in seven polio survivors to document objectively abnormal movements in sleep .
	manualset3
137940	4	407173	5	NULL	NULL	0	NULL	objectively abnormal movements	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep studies were performed in seven polio survivors to document objectively abnormal movements in sleep .
	manualset3
137941	5	407173	5	NULL	NULL	0	NULL	sleep 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep studies were performed in seven polio survivors to document objectively abnormal movements in sleep .
	manualset3
137942	1	407174	5	NULL	NULL	NULL	NULL	Slices 	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Slices of drone retina were superfused with a Ringer solution containing 1 mM tetraethylammonium ( TEA ) , and the concentration of this ion in the extracellular space ( ( TEA ) 0 ) was measured with ion-sensitive microelectrodes .
	manualset3
137943	2	407174	5	NULL	NULL	0	NULL	drone retina	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Slices of drone retina were superfused with a Ringer solution containing 1 mM tetraethylammonium ( TEA ) , and the concentration of this ion in the extracellular space ( ( TEA ) 0 ) was measured with ion-sensitive microelectrodes .
	manualset3
137944	3	407174	5	NULL	NULL	0	NULL	Ringer solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Slices of drone retina were superfused with a Ringer solution containing 1 mM tetraethylammonium ( TEA ) , and the concentration of this ion in the extracellular space ( ( TEA ) 0 ) was measured with ion-sensitive microelectrodes .
	manualset3
137945	4	407174	5	NULL	NULL	0	NULL	1 mM tetraethylammonium ( TEA )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Slices of drone retina were superfused with a Ringer solution containing 1 mM tetraethylammonium ( TEA ) , and the concentration of this ion in the extracellular space ( ( TEA ) 0 ) was measured with ion-sensitive microelectrodes .
	manualset3
137946	5	407174	5	NULL	NULL	0	NULL	concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Slices of drone retina were superfused with a Ringer solution containing 1 mM tetraethylammonium ( TEA ) , and the concentration of this ion in the extracellular space ( ( TEA ) 0 ) was measured with ion-sensitive microelectrodes .
	manualset3
137947	6	407174	5	NULL	NULL	0	NULL	ion 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Slices of drone retina were superfused with a Ringer solution containing 1 mM tetraethylammonium ( TEA ) , and the concentration of this ion in the extracellular space ( ( TEA ) 0 ) was measured with ion-sensitive microelectrodes .
	manualset3
137948	7	407174	5	NULL	NULL	0	NULL	extracellular space	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Slices of drone retina were superfused with a Ringer solution containing 1 mM tetraethylammonium ( TEA ) , and the concentration of this ion in the extracellular space ( ( TEA ) 0 ) was measured with ion-sensitive microelectrodes .
	manualset3
137949	8	407174	5	NULL	NULL	0	NULL	( ( TEA ) 0 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Slices of drone retina were superfused with a Ringer solution containing 1 mM tetraethylammonium ( TEA ) , and the concentration of this ion in the extracellular space ( ( TEA ) 0 ) was measured with ion-sensitive microelectrodes .
	manualset3
137950	9	407174	5	NULL	NULL	0	NULL	ion-sensitive microelectrodes	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Slices of drone retina were superfused with a Ringer solution containing 1 mM tetraethylammonium ( TEA ) , and the concentration of this ion in the extracellular space ( ( TEA ) 0 ) was measured with ion-sensitive microelectrodes .
	manualset3
137951	1	407175	5	NULL	NULL	NULL	NULL	Slit smears	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Slit smears form 16 LL and 4 BL patients were taken from scalp , axilla , inguinal regions and apparently involved skin patch .
	manualset3
137952	2	407175	5	NULL	NULL	0	NULL	16 LL patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Slit smears form 16 LL and 4 BL patients were taken from scalp , axilla , inguinal regions and apparently involved skin patch .
	manualset3
137953	3	407175	5	NULL	NULL	0	NULL	 4 BL patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Slit smears form 16 LL and 4 BL patients were taken from scalp , axilla , inguinal regions and apparently involved skin patch .
	manualset3
137954	4	407175	5	NULL	NULL	0	NULL	scalp 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Slit smears form 16 LL and 4 BL patients were taken from scalp , axilla , inguinal regions and apparently involved skin patch .
	manualset3
137955	5	407175	5	NULL	NULL	0	NULL	axilla 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Slit smears form 16 LL and 4 BL patients were taken from scalp , axilla , inguinal regions and apparently involved skin patch .
	manualset3
137956	6	407175	5	NULL	NULL	0	NULL	inguinal regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Slit smears form 16 LL and 4 BL patients were taken from scalp , axilla , inguinal regions and apparently involved skin patch .
	manualset3
137957	7	407175	5	NULL	NULL	0	NULL	skin patch	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Slit smears form 16 LL and 4 BL patients were taken from scalp , axilla , inguinal regions and apparently involved skin patch .
	manualset3
137958	1	407176	5	NULL	NULL	0	NULL	Slit3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Slit3 is the predominant ligand transcribed in the early mouse heart and is expressed in the ventral wall of the linear heart tube and subsequently in chamber but not in atrioventricular canal myocardium .
	manualset3
137959	2	407176	5	NULL	NULL	0	NULL	predominant ligand	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Slit3 is the predominant ligand transcribed in the early mouse heart and is expressed in the ventral wall of the linear heart tube and subsequently in chamber but not in atrioventricular canal myocardium .
	manualset3
137960	3	407176	5	NULL	NULL	0	NULL	early mouse heart	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Slit3 is the predominant ligand transcribed in the early mouse heart and is expressed in the ventral wall of the linear heart tube and subsequently in chamber but not in atrioventricular canal myocardium .
	manualset3
137961	4	407176	5	NULL	NULL	0	NULL	ventral wall	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Slit3 is the predominant ligand transcribed in the early mouse heart and is expressed in the ventral wall of the linear heart tube and subsequently in chamber but not in atrioventricular canal myocardium .
	manualset3
137962	5	407176	5	NULL	NULL	0	NULL	linear heart tube 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Slit3 is the predominant ligand transcribed in the early mouse heart and is expressed in the ventral wall of the linear heart tube and subsequently in chamber but not in atrioventricular canal myocardium .
	manualset3
137963	6	407176	5	NULL	NULL	0	NULL	chamber 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Slit3 is the predominant ligand transcribed in the early mouse heart and is expressed in the ventral wall of the linear heart tube and subsequently in chamber but not in atrioventricular canal myocardium .
	manualset3
137964	7	407176	5	NULL	NULL	0	NULL	atrioventricular canal myocardium	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Slit3 is the predominant ligand transcribed in the early mouse heart and is expressed in the ventral wall of the linear heart tube and subsequently in chamber but not in atrioventricular canal myocardium .
	manualset3
137965	1	407177	5	NULL	NULL	0	NULL	Slow bone resorption	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Slow bone resorption has been observed at the interface between the block and the surrounding bone , but the interproximal bone peaks , important for soft tissue support and esthetics , have been maintained over time .
	manualset3
137966	2	407177	5	NULL	NULL	0	NULL	interface 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Slow bone resorption has been observed at the interface between the block and the surrounding bone , but the interproximal bone peaks , important for soft tissue support and esthetics , have been maintained over time .
	manualset3
137967	3	407177	5	NULL	NULL	0	NULL	block 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Slow bone resorption has been observed at the interface between the block and the surrounding bone , but the interproximal bone peaks , important for soft tissue support and esthetics , have been maintained over time .
	manualset3
137968	4	407177	5	NULL	NULL	0	NULL	surrounding bone	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Slow bone resorption has been observed at the interface between the block and the surrounding bone , but the interproximal bone peaks , important for soft tissue support and esthetics , have been maintained over time .
	manualset3
137969	5	407177	5	NULL	NULL	0	NULL	interproximal bone peaks	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Slow bone resorption has been observed at the interface between the block and the surrounding bone , but the interproximal bone peaks , important for soft tissue support and esthetics , have been maintained over time .
	manualset3
137970	6	407177	5	NULL	NULL	0	NULL	soft tissue support 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Slow bone resorption has been observed at the interface between the block and the surrounding bone , but the interproximal bone peaks , important for soft tissue support and esthetics , have been maintained over time .
	manualset3
137971	7	407177	5	NULL	NULL	0	NULL	esthetics 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Slow bone resorption has been observed at the interface between the block and the surrounding bone , but the interproximal bone peaks , important for soft tissue support and esthetics , have been maintained over time .
	manualset3
137972	8	407177	5	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Slow bone resorption has been observed at the interface between the block and the surrounding bone , but the interproximal bone peaks , important for soft tissue support and esthetics , have been maintained over time .
	manualset3
137973	1	407178	5	NULL	NULL	0	NULL	Small-molecule inhibitors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Small-molecule inhibitors of the PI3K signaling network .
	manualset3
137974	2	407178	5	NULL	NULL	0	NULL	PI3K signaling network	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Small-molecule inhibitors of the PI3K signaling network .
	manualset3
137975	1	407179	5	NULL	NULL	0	NULL	Small ( SKCa ) Ca2 + - activated K + channels 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Small ( SKCa ) Ca2 + - activated K + channels were identified in membrane patches excised from cultured CA1-CA3 pyramidal neurones of the neonatal rat hippocampus .
	manualset3
137976	2	407179	5	NULL	NULL	0	NULL	membrane patches	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Small ( SKCa ) Ca2 + - activated K + channels were identified in membrane patches excised from cultured CA1-CA3 pyramidal neurones of the neonatal rat hippocampus .
	manualset3
137977	3	407179	5	NULL	NULL	0	NULL	cultured CA1-CA3 pyramidal neurones	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Small ( SKCa ) Ca2 + - activated K + channels were identified in membrane patches excised from cultured CA1-CA3 pyramidal neurones of the neonatal rat hippocampus .
	manualset3
137978	4	407179	5	NULL	NULL	0	NULL	neonatal rat hippocampus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Small ( SKCa ) Ca2 + - activated K + channels were identified in membrane patches excised from cultured CA1-CA3 pyramidal neurones of the neonatal rat hippocampus .
	manualset3
137979	1	407180	5	NULL	NULL	0	NULL	Small amounts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Small amounts of tissue from specific regions of the marmoset monkey brain were pretreated using solid-phase extraction as a clean-up and concentrating step .
	manualset3
137980	2	407180	5	NULL	NULL	0	NULL	tissue 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Small amounts of tissue from specific regions of the marmoset monkey brain were pretreated using solid-phase extraction as a clean-up and concentrating step .
	manualset3
137981	3	407180	5	NULL	NULL	0	NULL	specific regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Small amounts of tissue from specific regions of the marmoset monkey brain were pretreated using solid-phase extraction as a clean-up and concentrating step .
	manualset3
137982	4	407180	5	NULL	NULL	0	NULL	marmoset monkey brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Small amounts of tissue from specific regions of the marmoset monkey brain were pretreated using solid-phase extraction as a clean-up and concentrating step .
	manualset3
137983	5	407180	5	NULL	NULL	0	NULL	solid-phase extraction 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Small amounts of tissue from specific regions of the marmoset monkey brain were pretreated using solid-phase extraction as a clean-up and concentrating step .
	manualset3
137984	6	407180	5	NULL	NULL	0	NULL	clean-up	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Small amounts of tissue from specific regions of the marmoset monkey brain were pretreated using solid-phase extraction as a clean-up and concentrating step .
	manualset3
137985	7	407180	5	NULL	NULL	0	NULL	concentrating step	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Small amounts of tissue from specific regions of the marmoset monkey brain were pretreated using solid-phase extraction as a clean-up and concentrating step .
	manualset3
137986	1	407181	5	NULL	NULL	0	NULL	Small bowel tuberculosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Small bowel tuberculosis diagnosed by the combination of video capsule endoscopy and double balloon enteroscopy .
	manualset3
137987	2	407181	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Small bowel tuberculosis diagnosed by the combination of video capsule endoscopy and double balloon enteroscopy .
	manualset3
137988	3	407181	5	NULL	NULL	0	NULL	video capsule endoscopy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Small bowel tuberculosis diagnosed by the combination of video capsule endoscopy and double balloon enteroscopy .
	manualset3
137989	4	407181	5	NULL	NULL	0	NULL	double balloon enteroscopy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Small bowel tuberculosis diagnosed by the combination of video capsule endoscopy and double balloon enteroscopy .
	manualset3
137990	1	407182	5	NULL	NULL	0	NULL	Small children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Small children and infants were scanned inside a 32 cm diameter proton head coil .
	manualset3
137991	2	407182	5	NULL	NULL	0	NULL	infants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Small children and infants were scanned inside a 32 cm diameter proton head coil .
	manualset3
137992	3	407182	5	NULL	NULL	0	NULL	32 cm diameter proton head coil	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Small children and infants were scanned inside a 32 cm diameter proton head coil .
	manualset3
137993	1	407183	5	NULL	NULL	0	NULL	differences 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Small differences in response may be obliterated by using excessive concentrations of a given reagent .
	manualset3
137994	2	407183	5	NULL	NULL	0	NULL	response 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Small differences in response may be obliterated by using excessive concentrations of a given reagent .
	manualset3
137995	3	407183	5	NULL	NULL	0	NULL	excessive concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Small differences in response may be obliterated by using excessive concentrations of a given reagent .
	manualset3
137996	4	407183	5	NULL	NULL	0	NULL	reagent 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Small differences in response may be obliterated by using excessive concentrations of a given reagent .
	manualset3
137997	1	407184	5	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of transcripts bearing homology to retroviral elements that were detected add to a growing body of evidence for extensive invasion of errantiviruses into the insect genome .
	manualset3
137998	2	407184	5	NULL	NULL	0	NULL	transcripts 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of transcripts bearing homology to retroviral elements that were detected add to a growing body of evidence for extensive invasion of errantiviruses into the insect genome .
	manualset3
137999	3	407184	5	NULL	NULL	0	NULL	homology 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of transcripts bearing homology to retroviral elements that were detected add to a growing body of evidence for extensive invasion of errantiviruses into the insect genome .
	manualset3
138000	4	407184	5	NULL	NULL	0	NULL	retroviral elements 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of transcripts bearing homology to retroviral elements that were detected add to a growing body of evidence for extensive invasion of errantiviruses into the insect genome .
	manualset3
138001	5	407184	5	NULL	NULL	0	NULL	growing body of evidence	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of transcripts bearing homology to retroviral elements that were detected add to a growing body of evidence for extensive invasion of errantiviruses into the insect genome .
	manualset3
138002	6	407184	5	NULL	NULL	0	NULL	extensive invasion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of transcripts bearing homology to retroviral elements that were detected add to a growing body of evidence for extensive invasion of errantiviruses into the insect genome .
	manualset3
138003	7	407184	5	NULL	NULL	0	NULL	errantiviruses 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of transcripts bearing homology to retroviral elements that were detected add to a growing body of evidence for extensive invasion of errantiviruses into the insect genome .
	manualset3
138004	8	407184	5	NULL	NULL	0	NULL	insect genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of transcripts bearing homology to retroviral elements that were detected add to a growing body of evidence for extensive invasion of errantiviruses into the insect genome .
	manualset3
138005	1	407185	5	NULL	NULL	0	NULL	Small doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Small doses of radiotherapy ( 10-20 Gy in 5-10 fractions ) relieved symptoms in all of these patients .
	manualset3
138006	2	407185	5	NULL	NULL	0	NULL	radiotherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Small doses of radiotherapy ( 10-20 Gy in 5-10 fractions ) relieved symptoms in all of these patients .
	manualset3
138007	3	407185	5	NULL	NULL	0	NULL	10-20 Gy in 5-10 fractions	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Small doses of radiotherapy ( 10-20 Gy in 5-10 fractions ) relieved symptoms in all of these patients .
	manualset3
138008	4	407185	5	NULL	NULL	NULL	NULL	symptoms 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Small doses of radiotherapy ( 10-20 Gy in 5-10 fractions ) relieved symptoms in all of these patients .
	manualset3
138009	5	407185	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Small doses of radiotherapy ( 10-20 Gy in 5-10 fractions ) relieved symptoms in all of these patients .
	manualset3
138010	1	407186	5	NULL	NULL	0	NULL	Small lower pole stones	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Small lower pole stones & lt ; 1cm can be monitored actively .
	manualset3
138011	2	407186	5	NULL	NULL	0	NULL	 & lt ; 1cm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Small lower pole stones & lt ; 1cm can be monitored actively .
	manualset3
138012	1	407187	5	NULL	NULL	0	NULL	Small molecular weight variants of p53 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Small molecular weight variants of p53 are expressed in human melanoma cells and are induced by the DNA-damaging agent cisplatin .
	manualset3
138013	2	407187	5	NULL	NULL	0	NULL	human melanoma cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Small molecular weight variants of p53 are expressed in human melanoma cells and are induced by the DNA-damaging agent cisplatin .
	manualset3
138014	3	407187	5	NULL	NULL	0	NULL	DNA-damaging agent cisplatin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Small molecular weight variants of p53 are expressed in human melanoma cells and are induced by the DNA-damaging agent cisplatin .
	manualset3
138015	1	407188	5	NULL	NULL	0	NULL	Small tooth sizes 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Small tooth sizes in a nineteenth century South Carolina plantation slave series .
	manualset3
138016	2	407188	5	NULL	NULL	0	NULL	nineteenth century South Carolina plantation slave series	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Small tooth sizes in a nineteenth century South Carolina plantation slave series .
	manualset3
138017	1	407189	5	NULL	NULL	0	NULL	Smears 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Smears of B. bovis-infected blood were used as the source of antigen in the test which was read using a light microscope .
	manualset3
138018	2	407189	5	NULL	NULL	0	NULL	B. bovis-infected blood 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Smears of B. bovis-infected blood were used as the source of antigen in the test which was read using a light microscope .
	manualset3
138019	3	407189	5	NULL	NULL	0	NULL	source 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Smears of B. bovis-infected blood were used as the source of antigen in the test which was read using a light microscope .
	manualset3
138020	4	407189	5	NULL	NULL	0	NULL	antigen 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Smears of B. bovis-infected blood were used as the source of antigen in the test which was read using a light microscope .
	manualset3
138021	5	407189	5	NULL	NULL	0	NULL	test 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Smears of B. bovis-infected blood were used as the source of antigen in the test which was read using a light microscope .
	manualset3
138022	6	407189	5	NULL	NULL	0	NULL	light microscope	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Smears of B. bovis-infected blood were used as the source of antigen in the test which was read using a light microscope .
	manualset3
138023	1	407190	5	NULL	NULL	0	NULL	Smoke exposure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Smoke exposure with BH regularly produced severe injury in terms of decreased PaO2 and histopathologic changes , while exposure without BH did not , despite high levels of carboxyhemoglobin after smoke inhalation .
	manualset3
138024	2	407190	5	NULL	NULL	0	NULL	BH 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Smoke exposure with BH regularly produced severe injury in terms of decreased PaO2 and histopathologic changes , while exposure without BH did not , despite high levels of carboxyhemoglobin after smoke inhalation .
	manualset3
138025	3	407190	5	NULL	NULL	0	NULL	severe injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Smoke exposure with BH regularly produced severe injury in terms of decreased PaO2 and histopathologic changes , while exposure without BH did not , despite high levels of carboxyhemoglobin after smoke inhalation .
	manualset3
138026	4	407190	5	NULL	NULL	0	NULL	PaO2 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Smoke exposure with BH regularly produced severe injury in terms of decreased PaO2 and histopathologic changes , while exposure without BH did not , despite high levels of carboxyhemoglobin after smoke inhalation .
	manualset3
138027	5	407190	5	NULL	NULL	0	NULL	histopathologic changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Smoke exposure with BH regularly produced severe injury in terms of decreased PaO2 and histopathologic changes , while exposure without BH did not , despite high levels of carboxyhemoglobin after smoke inhalation .
	manualset3
138028	6	407190	5	NULL	NULL	0	NULL	exposure 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Smoke exposure with BH regularly produced severe injury in terms of decreased PaO2 and histopathologic changes , while exposure without BH did not , despite high levels of carboxyhemoglobin after smoke inhalation .
	manualset3
138029	7	407190	5	NULL	NULL	0	NULL	BH 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Smoke exposure with BH regularly produced severe injury in terms of decreased PaO2 and histopathologic changes , while exposure without BH did not , despite high levels of carboxyhemoglobin after smoke inhalation .
	manualset3
138030	8	407190	5	NULL	NULL	0	NULL	high levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Smoke exposure with BH regularly produced severe injury in terms of decreased PaO2 and histopathologic changes , while exposure without BH did not , despite high levels of carboxyhemoglobin after smoke inhalation .
	manualset3
138031	9	407190	5	NULL	NULL	0	NULL	carboxyhemoglobin 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Smoke exposure with BH regularly produced severe injury in terms of decreased PaO2 and histopathologic changes , while exposure without BH did not , despite high levels of carboxyhemoglobin after smoke inhalation .
	manualset3
138032	10	407190	5	NULL	NULL	0	NULL	smoke inhalation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Smoke exposure with BH regularly produced severe injury in terms of decreased PaO2 and histopathologic changes , while exposure without BH did not , despite high levels of carboxyhemoglobin after smoke inhalation .
	manualset3
138033	1	407191	5	NULL	NULL	0	NULL	Smoking cessation attempts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Smoking cessation attempts among adolescent smokers : a systematic review of prevalence studies .
	manualset3
138034	2	407191	5	NULL	NULL	0	NULL	adolescent smokers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Smoking cessation attempts among adolescent smokers : a systematic review of prevalence studies .
	manualset3
138035	3	407191	5	NULL	NULL	0	NULL	systematic review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Smoking cessation attempts among adolescent smokers : a systematic review of prevalence studies .
	manualset3
138036	4	407191	5	NULL	NULL	0	NULL	prevalence studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Smoking cessation attempts among adolescent smokers : a systematic review of prevalence studies .
	manualset3
138037	1	407192	5	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of transformants reverted to a flat , `` normal '' morphology shortly after isolation .
	manualset3
138038	2	407192	5	NULL	NULL	NULL	NULL	transformants 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A number of transformants reverted to a flat , `` normal '' morphology shortly after isolation .
	manualset3
138039	3	407192	5	NULL	NULL	0	NULL	 flat , `` normal '' morphology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of transformants reverted to a flat , `` normal '' morphology shortly after isolation .
	manualset3
138040	4	407192	5	NULL	NULL	0	NULL	isolation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of transformants reverted to a flat , `` normal '' morphology shortly after isolation .
	manualset3
138041	1	407193	5	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	So it can be clearly stated that increase in the free radical by hyperglycemia , lipid peroxidation and advanced glycosylation endproducts along with decreased antioxidants are the causative agents for the development of retinopathy .
	manualset3
138042	2	407193	5	NULL	NULL	0	NULL	free radical	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	So it can be clearly stated that increase in the free radical by hyperglycemia , lipid peroxidation and advanced glycosylation endproducts along with decreased antioxidants are the causative agents for the development of retinopathy .
	manualset3
138043	3	407193	5	NULL	NULL	0	NULL	hyperglycemia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	So it can be clearly stated that increase in the free radical by hyperglycemia , lipid peroxidation and advanced glycosylation endproducts along with decreased antioxidants are the causative agents for the development of retinopathy .
	manualset3
138044	4	407193	5	NULL	NULL	0	NULL	lipid peroxidation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	So it can be clearly stated that increase in the free radical by hyperglycemia , lipid peroxidation and advanced glycosylation endproducts along with decreased antioxidants are the causative agents for the development of retinopathy .
	manualset3
138045	5	407193	5	NULL	NULL	0	NULL	advanced glycosylation endproducts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	So it can be clearly stated that increase in the free radical by hyperglycemia , lipid peroxidation and advanced glycosylation endproducts along with decreased antioxidants are the causative agents for the development of retinopathy .
	manualset3
138046	6	407193	5	NULL	NULL	0	NULL	antioxidants 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	So it can be clearly stated that increase in the free radical by hyperglycemia , lipid peroxidation and advanced glycosylation endproducts along with decreased antioxidants are the causative agents for the development of retinopathy .
	manualset3
138047	7	407193	5	NULL	NULL	0	NULL	causative agents 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	So it can be clearly stated that increase in the free radical by hyperglycemia , lipid peroxidation and advanced glycosylation endproducts along with decreased antioxidants are the causative agents for the development of retinopathy .
	manualset3
138048	8	407193	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	So it can be clearly stated that increase in the free radical by hyperglycemia , lipid peroxidation and advanced glycosylation endproducts along with decreased antioxidants are the causative agents for the development of retinopathy .
	manualset3
138049	9	407193	5	NULL	NULL	0	NULL	retinopathy 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	So it can be clearly stated that increase in the free radical by hyperglycemia , lipid peroxidation and advanced glycosylation endproducts along with decreased antioxidants are the causative agents for the development of retinopathy .
	manualset3
138050	1	407194	5	NULL	NULL	0	NULL	countermeasure factor	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	So called `` countermeasure factor '' was used for specification of other model results .
	manualset3
138051	2	407194	5	NULL	NULL	0	NULL	specification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	So called `` countermeasure factor '' was used for specification of other model results .
	manualset3
138052	3	407194	5	NULL	NULL	0	NULL	model results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	So called `` countermeasure factor '' was used for specification of other model results .
	manualset3
138053	1	407195	5	NULL	NULL	0	NULL	MAD2L2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	So far , MAD2L2 has not been reported to play a major role in human cancer in contrast to its homolog MAD2 .
	manualset3
138054	2	407195	5	NULL	NULL	0	NULL	major role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	So far , MAD2L2 has not been reported to play a major role in human cancer in contrast to its homolog MAD2 .
	manualset3
138055	3	407195	5	NULL	NULL	0	NULL	human cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	So far , MAD2L2 has not been reported to play a major role in human cancer in contrast to its homolog MAD2 .
	manualset3
138056	4	407195	5	NULL	NULL	0	NULL	homolog MAD2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	So far , MAD2L2 has not been reported to play a major role in human cancer in contrast to its homolog MAD2 .
	manualset3
138057	1	407196	5	NULL	NULL	0	NULL	2 , 300	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	So far , over 2 , 300 , 500 , and 80 Alu , L1 , and SVA insertions , respectively , have been reported to be polymorphic and many more are yet to be discovered .
	manualset3
138058	2	407196	5	NULL	NULL	0	NULL	500 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	So far , over 2 , 300 , 500 , and 80 Alu , L1 , and SVA insertions , respectively , have been reported to be polymorphic and many more are yet to be discovered .
	manualset3
138059	3	407196	5	NULL	NULL	0	NULL	80 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	So far , over 2 , 300 , 500 , and 80 Alu , L1 , and SVA insertions , respectively , have been reported to be polymorphic and many more are yet to be discovered .
	manualset3
138060	4	407196	5	NULL	NULL	0	NULL	Alu insertions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	So far , over 2 , 300 , 500 , and 80 Alu , L1 , and SVA insertions , respectively , have been reported to be polymorphic and many more are yet to be discovered .
	manualset3
138061	5	407196	5	NULL	NULL	0	NULL	L1 insertions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	So far , over 2 , 300 , 500 , and 80 Alu , L1 , and SVA insertions , respectively , have been reported to be polymorphic and many more are yet to be discovered .
	manualset3
138062	6	407196	5	NULL	NULL	0	NULL	SVA insertions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	So far , over 2 , 300 , 500 , and 80 Alu , L1 , and SVA insertions , respectively , have been reported to be polymorphic and many more are yet to be discovered .
	manualset3
138063	1	407197	5	NULL	NULL	0	NULL	three 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	So far , three drugs have been approved for the treatment of anemia in patients with malignancies ( epoetin alfa , epoetin beta and darbepoetin alfa ) .
	manualset3
138064	2	407197	5	NULL	NULL	0	NULL	drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	So far , three drugs have been approved for the treatment of anemia in patients with malignancies ( epoetin alfa , epoetin beta and darbepoetin alfa ) .
	manualset3
138065	3	407197	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	So far , three drugs have been approved for the treatment of anemia in patients with malignancies ( epoetin alfa , epoetin beta and darbepoetin alfa ) .
	manualset3
138066	4	407197	5	NULL	NULL	0	NULL	anemia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	So far , three drugs have been approved for the treatment of anemia in patients with malignancies ( epoetin alfa , epoetin beta and darbepoetin alfa ) .
	manualset3
138067	5	407197	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	So far , three drugs have been approved for the treatment of anemia in patients with malignancies ( epoetin alfa , epoetin beta and darbepoetin alfa ) .
	manualset3
138068	6	407197	5	NULL	NULL	0	NULL	malignancies 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	So far , three drugs have been approved for the treatment of anemia in patients with malignancies ( epoetin alfa , epoetin beta and darbepoetin alfa ) .
	manualset3
138069	7	407197	5	NULL	NULL	0	NULL	epoetin alfa	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	So far , three drugs have been approved for the treatment of anemia in patients with malignancies ( epoetin alfa , epoetin beta and darbepoetin alfa ) .
	manualset3
138070	8	407197	5	NULL	NULL	0	NULL	epoetin beta	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	So far , three drugs have been approved for the treatment of anemia in patients with malignancies ( epoetin alfa , epoetin beta and darbepoetin alfa ) .
	manualset3
138071	9	407197	5	NULL	NULL	0	NULL	darbepoetin alfa	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	So far , three drugs have been approved for the treatment of anemia in patients with malignancies ( epoetin alfa , epoetin beta and darbepoetin alfa ) .
	manualset3
138072	1	407198	5	NULL	NULL	0	NULL	neuroprotection 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	So we suggest that this neuroprotection may not be related to depression of iNOS expression .
	manualset3
138073	2	407198	5	NULL	NULL	0	NULL	depression 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	So we suggest that this neuroprotection may not be related to depression of iNOS expression .
	manualset3
138074	3	407198	5	NULL	NULL	0	NULL	iNOS expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	So we suggest that this neuroprotection may not be related to depression of iNOS expression .
	manualset3
138075	1	407199	5	NULL	NULL	0	NULL	Social implications 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Social and ethical implications of genomics , race , ethnicity , and health inequities .
	manualset3
138076	2	407199	5	NULL	NULL	0	NULL	ethical implications 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Social and ethical implications of genomics , race , ethnicity , and health inequities .
	manualset3
138077	3	407199	5	NULL	NULL	NULL	NULL	genomics inequities 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Social and ethical implications of genomics , race , ethnicity , and health inequities .
	manualset3
138078	4	407199	5	NULL	NULL	NULL	NULL	race inequities 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Social and ethical implications of genomics , race , ethnicity , and health inequities .
	manualset3
138079	5	407199	5	NULL	NULL	NULL	NULL	ethnicity inequities 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Social and ethical implications of genomics , race , ethnicity , and health inequities .
	manualset3
138080	6	407199	5	NULL	NULL	0	NULL	health inequities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Social and ethical implications of genomics , race , ethnicity , and health inequities .
	manualset3
138081	1	407200	5	NULL	NULL	0	NULL	Social aspects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Social aspects of palliation can be divided into two major areas -- social counselling and psycho-social work .
	manualset3
138082	2	407200	5	NULL	NULL	0	NULL	palliation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Social aspects of palliation can be divided into two major areas -- social counselling and psycho-social work .
	manualset3
138083	3	407200	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Social aspects of palliation can be divided into two major areas -- social counselling and psycho-social work .
	manualset3
138084	4	407200	5	NULL	NULL	0	NULL	major areas	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Social aspects of palliation can be divided into two major areas -- social counselling and psycho-social work .
	manualset3
138085	5	407200	5	NULL	NULL	NULL	NULL	social counselling	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Social aspects of palliation can be divided into two major areas -- social counselling and psycho-social work .
	manualset3
138086	6	407200	5	NULL	NULL	0	NULL	psycho-social work	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Social aspects of palliation can be divided into two major areas -- social counselling and psycho-social work .
	manualset3
138087	1	407201	5	NULL	NULL	0	NULL	Social scientific studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Social scientific and nursing studies , and the experiences of emergency department staff , have attested to the complex organisational and communicative work that accompanies emergency clinical work .
	manualset3
138088	2	407201	5	NULL	NULL	0	NULL	nursing studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Social scientific and nursing studies , and the experiences of emergency department staff , have attested to the complex organisational and communicative work that accompanies emergency clinical work .
	manualset3
138089	3	407201	5	NULL	NULL	0	NULL	experiences 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Social scientific and nursing studies , and the experiences of emergency department staff , have attested to the complex organisational and communicative work that accompanies emergency clinical work .
	manualset3
138090	4	407201	5	NULL	NULL	0	NULL	emergency department staff	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Social scientific and nursing studies , and the experiences of emergency department staff , have attested to the complex organisational and communicative work that accompanies emergency clinical work .
	manualset3
138091	5	407201	5	NULL	NULL	0	NULL	complex organisational and communicative work	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Social scientific and nursing studies , and the experiences of emergency department staff , have attested to the complex organisational and communicative work that accompanies emergency clinical work .
	manualset3
138092	6	407201	5	NULL	NULL	0	NULL	emergency clinical work	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Social scientific and nursing studies , and the experiences of emergency department staff , have attested to the complex organisational and communicative work that accompanies emergency clinical work .
	manualset3
138093	1	407202	5	NULL	NULL	0	NULL	Social support	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Social support indirectly predicted physical activity through its effect on self-efficacy .
	manualset3
138094	2	407202	5	NULL	NULL	0	NULL	physical activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Social support indirectly predicted physical activity through its effect on self-efficacy .
	manualset3
138095	3	407202	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Social support indirectly predicted physical activity through its effect on self-efficacy .
	manualset3
138096	4	407202	5	NULL	NULL	0	NULL	self-efficacy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Social support indirectly predicted physical activity through its effect on self-efficacy .
	manualset3
138097	1	407203	5	NULL	NULL	0	NULL	Social work practice 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Social work practice in health care : looking to the future with a different lens .
	manualset3
138098	2	407203	5	NULL	NULL	0	NULL	health care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Social work practice in health care : looking to the future with a different lens .
	manualset3
138099	3	407203	5	NULL	NULL	0	NULL	future 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Social work practice in health care : looking to the future with a different lens .
	manualset3
138100	4	407203	5	NULL	NULL	0	NULL	different lens	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Social work practice in health care : looking to the future with a different lens .
	manualset3
138101	1	407204	5	NULL	NULL	0	NULL	Social networks	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Social networks and recovery : one year after inpatient treatment .
	manualset3
138102	2	407204	5	NULL	NULL	0	NULL	recovery 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Social networks and recovery : one year after inpatient treatment .
	manualset3
138103	3	407204	5	NULL	NULL	0	NULL	one year	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Social networks and recovery : one year after inpatient treatment .
	manualset3
138104	4	407204	5	NULL	NULL	0	NULL	inpatient treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Social networks and recovery : one year after inpatient treatment .
	manualset3
138105	1	407205	5	NULL	NULL	0	NULL	Social support	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Social support was based on self-reports of access to support from relatives and friends .
	manualset3
138106	2	407205	5	NULL	NULL	0	NULL	self-reports 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Social support was based on self-reports of access to support from relatives and friends .
	manualset3
138107	3	407205	5	NULL	NULL	0	NULL	support 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Social support was based on self-reports of access to support from relatives and friends .
	manualset3
138108	4	407205	5	NULL	NULL	0	NULL	relatives 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Social support was based on self-reports of access to support from relatives and friends .
	manualset3
138109	5	407205	5	NULL	NULL	0	NULL	friends 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Social support was based on self-reports of access to support from relatives and friends .
	manualset3
138110	1	407206	5	NULL	NULL	0	NULL	Socially deprived monkeys 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Socially deprived monkeys showed higher rates of submission and stereotypic behaviors than socially reared individuals .
	manualset3
138111	2	407206	5	NULL	NULL	0	NULL	higher rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Socially deprived monkeys showed higher rates of submission and stereotypic behaviors than socially reared individuals .
	manualset3
138112	3	407206	5	NULL	NULL	0	NULL	submission 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Socially deprived monkeys showed higher rates of submission and stereotypic behaviors than socially reared individuals .
	manualset3
138113	4	407206	5	NULL	NULL	0	NULL	stereotypic behaviors	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Socially deprived monkeys showed higher rates of submission and stereotypic behaviors than socially reared individuals .
	manualset3
138114	5	407206	5	NULL	NULL	0	NULL	socially reared individuals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Socially deprived monkeys showed higher rates of submission and stereotypic behaviors than socially reared individuals .
	manualset3
138115	1	407207	5	NULL	NULL	0	NULL	nurse-supervised exercise stress testing laboratory	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A nurse-supervised exercise stress testing laboratory .
	manualset3
138116	1	407208	5	NULL	NULL	0	NULL	Socio-economic and household information 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Socio-economic and household information was obtained by interview and observation .
	manualset3
138117	2	407208	5	NULL	NULL	0	NULL	interview 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Socio-economic and household information was obtained by interview and observation .
	manualset3
138118	3	407208	5	NULL	NULL	0	NULL	observation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Socio-economic and household information was obtained by interview and observation .
	manualset3
138119	1	407209	5	NULL	NULL	0	NULL	Sodium arsanilate	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium arsanilate is one of the most commonly used substances for chemical vestibular lesioning , but it is not well described in the literature .
	manualset3
138120	2	407209	5	NULL	NULL	0	NULL	substances 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium arsanilate is one of the most commonly used substances for chemical vestibular lesioning , but it is not well described in the literature .
	manualset3
138121	3	407209	5	NULL	NULL	0	NULL	chemical vestibular lesioning	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium arsanilate is one of the most commonly used substances for chemical vestibular lesioning , but it is not well described in the literature .
	manualset3
138122	4	407209	5	NULL	NULL	0	NULL	literature 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium arsanilate is one of the most commonly used substances for chemical vestibular lesioning , but it is not well described in the literature .
	manualset3
138123	1	407210	5	NULL	NULL	0	NULL	Sodium ascorbyl phosphate ( SAP )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium ascorbyl phosphate ( SAP ) represents a stable precursor of vitamin C that ensures a constant delivery of vitamin C into the skin .
	manualset3
138124	2	407210	5	NULL	NULL	0	NULL	stable precursor	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium ascorbyl phosphate ( SAP ) represents a stable precursor of vitamin C that ensures a constant delivery of vitamin C into the skin .
	manualset3
138125	3	407210	5	NULL	NULL	0	NULL	vitamin C	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium ascorbyl phosphate ( SAP ) represents a stable precursor of vitamin C that ensures a constant delivery of vitamin C into the skin .
	manualset3
138126	4	407210	5	NULL	NULL	0	NULL	constant delivery 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium ascorbyl phosphate ( SAP ) represents a stable precursor of vitamin C that ensures a constant delivery of vitamin C into the skin .
	manualset3
138127	5	407210	5	NULL	NULL	0	NULL	vitamin C	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium ascorbyl phosphate ( SAP ) represents a stable precursor of vitamin C that ensures a constant delivery of vitamin C into the skin .
	manualset3
138128	6	407210	5	NULL	NULL	0	NULL	skin 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium ascorbyl phosphate ( SAP ) represents a stable precursor of vitamin C that ensures a constant delivery of vitamin C into the skin .
	manualset3
138129	1	407211	5	NULL	NULL	0	NULL	Sodium channel ionic current ( INa ) 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium channel ionic current ( INa ) and gating current ( Ig ) were compared for rat skeletal ( rSkM1 ) and human heart Na + channels ( hH1a ) heterologously expressed in cultured mammalian cells at approximately 13 C before and after modification by site-3 toxins ( Anthopleurin A and Anthopleurin B ) .
	manualset3
138130	2	407211	5	NULL	NULL	0	NULL	gating current ( Ig ) 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium channel ionic current ( INa ) and gating current ( Ig ) were compared for rat skeletal ( rSkM1 ) and human heart Na + channels ( hH1a ) heterologously expressed in cultured mammalian cells at approximately 13 C before and after modification by site-3 toxins ( Anthopleurin A and Anthopleurin B ) .
	manualset3
138131	3	407211	5	NULL	NULL	0	NULL	rat skeletal ( rSkM1 )  Na + channels 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium channel ionic current ( INa ) and gating current ( Ig ) were compared for rat skeletal ( rSkM1 ) and human heart Na + channels ( hH1a ) heterologously expressed in cultured mammalian cells at approximately 13 C before and after modification by site-3 toxins ( Anthopleurin A and Anthopleurin B ) .
	manualset3
138132	4	407211	5	NULL	NULL	0	NULL	human heart Na + channels ( hH1a 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium channel ionic current ( INa ) and gating current ( Ig ) were compared for rat skeletal ( rSkM1 ) and human heart Na + channels ( hH1a ) heterologously expressed in cultured mammalian cells at approximately 13 C before and after modification by site-3 toxins ( Anthopleurin A and Anthopleurin B ) .
	manualset3
138133	5	407211	5	NULL	NULL	0	NULL	cultured mammalian cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium channel ionic current ( INa ) and gating current ( Ig ) were compared for rat skeletal ( rSkM1 ) and human heart Na + channels ( hH1a ) heterologously expressed in cultured mammalian cells at approximately 13 C before and after modification by site-3 toxins ( Anthopleurin A and Anthopleurin B ) .
	manualset3
138134	6	407211	5	NULL	NULL	0	NULL	13 C	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium channel ionic current ( INa ) and gating current ( Ig ) were compared for rat skeletal ( rSkM1 ) and human heart Na + channels ( hH1a ) heterologously expressed in cultured mammalian cells at approximately 13 C before and after modification by site-3 toxins ( Anthopleurin A and Anthopleurin B ) .
	manualset3
138135	7	407211	5	NULL	NULL	0	NULL	modification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium channel ionic current ( INa ) and gating current ( Ig ) were compared for rat skeletal ( rSkM1 ) and human heart Na + channels ( hH1a ) heterologously expressed in cultured mammalian cells at approximately 13 C before and after modification by site-3 toxins ( Anthopleurin A and Anthopleurin B ) .
	manualset3
138136	8	407211	5	NULL	NULL	0	NULL	site-3 toxins	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium channel ionic current ( INa ) and gating current ( Ig ) were compared for rat skeletal ( rSkM1 ) and human heart Na + channels ( hH1a ) heterologously expressed in cultured mammalian cells at approximately 13 C before and after modification by site-3 toxins ( Anthopleurin A and Anthopleurin B ) .
	manualset3
138137	9	407211	5	NULL	NULL	0	NULL	Anthopleurin A 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium channel ionic current ( INa ) and gating current ( Ig ) were compared for rat skeletal ( rSkM1 ) and human heart Na + channels ( hH1a ) heterologously expressed in cultured mammalian cells at approximately 13 C before and after modification by site-3 toxins ( Anthopleurin A and Anthopleurin B ) .
	manualset3
138138	10	407211	5	NULL	NULL	0	NULL	Anthopleurin B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium channel ionic current ( INa ) and gating current ( Ig ) were compared for rat skeletal ( rSkM1 ) and human heart Na + channels ( hH1a ) heterologously expressed in cultured mammalian cells at approximately 13 C before and after modification by site-3 toxins ( Anthopleurin A and Anthopleurin B ) .
	manualset3
138139	1	407212	5	NULL	NULL	0	NULL	Sodium dodecyl sulfate-polyacrylamide gel electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium dodecyl sulfate-polyacrylamide gel electrophoresis and western blotting comparisons of purified myofibrils and whole muscle preparations for evaluating titin and nebulin in postmortem bovine muscle .
	manualset3
138140	2	407212	5	NULL	NULL	0	NULL	western blotting	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium dodecyl sulfate-polyacrylamide gel electrophoresis and western blotting comparisons of purified myofibrils and whole muscle preparations for evaluating titin and nebulin in postmortem bovine muscle .
	manualset3
138141	3	407212	5	NULL	NULL	0	NULL	comparisons 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium dodecyl sulfate-polyacrylamide gel electrophoresis and western blotting comparisons of purified myofibrils and whole muscle preparations for evaluating titin and nebulin in postmortem bovine muscle .
	manualset3
138142	4	407212	5	NULL	NULL	0	NULL	purified myofibrils	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium dodecyl sulfate-polyacrylamide gel electrophoresis and western blotting comparisons of purified myofibrils and whole muscle preparations for evaluating titin and nebulin in postmortem bovine muscle .
	manualset3
138143	5	407212	5	NULL	NULL	0	NULL	whole muscle preparations	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium dodecyl sulfate-polyacrylamide gel electrophoresis and western blotting comparisons of purified myofibrils and whole muscle preparations for evaluating titin and nebulin in postmortem bovine muscle .
	manualset3
138144	6	407212	5	NULL	NULL	0	NULL	titin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium dodecyl sulfate-polyacrylamide gel electrophoresis and western blotting comparisons of purified myofibrils and whole muscle preparations for evaluating titin and nebulin in postmortem bovine muscle .
	manualset3
138145	7	407212	5	NULL	NULL	0	NULL	nebulin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium dodecyl sulfate-polyacrylamide gel electrophoresis and western blotting comparisons of purified myofibrils and whole muscle preparations for evaluating titin and nebulin in postmortem bovine muscle .
	manualset3
138146	8	407212	5	NULL	NULL	0	NULL	postmortem bovine muscle	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium dodecyl sulfate-polyacrylamide gel electrophoresis and western blotting comparisons of purified myofibrils and whole muscle preparations for evaluating titin and nebulin in postmortem bovine muscle .
	manualset3
138147	1	407213	5	NULL	NULL	0	NULL	Sodium dodecyl sulfate-polyacrylamide gel electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium dodecyl sulfate-polyacrylamide gel electrophoresis of HMG proteins revealed the presence of HMGs 1 and 2 as well as a 38 , 000-dalton protein .
	manualset3
138148	2	407213	5	NULL	NULL	0	NULL	HMG proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium dodecyl sulfate-polyacrylamide gel electrophoresis of HMG proteins revealed the presence of HMGs 1 and 2 as well as a 38 , 000-dalton protein .
	manualset3
138149	3	407213	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium dodecyl sulfate-polyacrylamide gel electrophoresis of HMG proteins revealed the presence of HMGs 1 and 2 as well as a 38 , 000-dalton protein .
	manualset3
138150	4	407213	5	NULL	NULL	0	NULL	HMG 1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium dodecyl sulfate-polyacrylamide gel electrophoresis of HMG proteins revealed the presence of HMGs 1 and 2 as well as a 38 , 000-dalton protein .
	manualset3
138151	5	407213	5	NULL	NULL	0	NULL	HMG 2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium dodecyl sulfate-polyacrylamide gel electrophoresis of HMG proteins revealed the presence of HMGs 1 and 2 as well as a 38 , 000-dalton protein .
	manualset3
138152	6	407213	5	NULL	NULL	0	NULL	38 , 000-dalton protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium dodecyl sulfate-polyacrylamide gel electrophoresis of HMG proteins revealed the presence of HMGs 1 and 2 as well as a 38 , 000-dalton protein .
	manualset3
138153	1	407214	5	NULL	NULL	0	NULL	Sodium dodecyl sulfate polyacrylamide gel electrophoresis results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium dodecyl sulfate polyacrylamide gel electrophoresis results showed that native and modified phospholipases B had exactly the same molecular weight ( 90 000 ) in the absence of beta-mercaptoethanol .
	manualset3
138154	2	407214	5	NULL	NULL	0	NULL	native phospholipases B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium dodecyl sulfate polyacrylamide gel electrophoresis results showed that native and modified phospholipases B had exactly the same molecular weight ( 90 000 ) in the absence of beta-mercaptoethanol .
	manualset3
138155	3	407214	5	NULL	NULL	0	NULL	modified phospholipases B 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium dodecyl sulfate polyacrylamide gel electrophoresis results showed that native and modified phospholipases B had exactly the same molecular weight ( 90 000 ) in the absence of beta-mercaptoethanol .
	manualset3
138156	4	407214	5	NULL	NULL	0	NULL	same molecular weight 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium dodecyl sulfate polyacrylamide gel electrophoresis results showed that native and modified phospholipases B had exactly the same molecular weight ( 90 000 ) in the absence of beta-mercaptoethanol .
	manualset3
138157	5	407214	5	NULL	NULL	0	NULL	 90 000	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium dodecyl sulfate polyacrylamide gel electrophoresis results showed that native and modified phospholipases B had exactly the same molecular weight ( 90 000 ) in the absence of beta-mercaptoethanol .
	manualset3
138158	6	407214	5	NULL	NULL	0	NULL	absence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium dodecyl sulfate polyacrylamide gel electrophoresis results showed that native and modified phospholipases B had exactly the same molecular weight ( 90 000 ) in the absence of beta-mercaptoethanol .
	manualset3
138159	7	407214	5	NULL	NULL	0	NULL	beta-mercaptoethanol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium dodecyl sulfate polyacrylamide gel electrophoresis results showed that native and modified phospholipases B had exactly the same molecular weight ( 90 000 ) in the absence of beta-mercaptoethanol .
	manualset3
138160	1	407215	5	NULL	NULL	0	NULL	Cerebral blood flow	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cerebral blood flow changes after mild head trauma imaging with SPECT HMPAO .
	manualset3
138161	2	407215	5	NULL	NULL	NULL	NULL	mild head trauma imaging	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Cerebral blood flow changes after mild head trauma imaging with SPECT HMPAO .
	manualset3
138162	3	407215	5	NULL	NULL	0	NULL	SPECT HMPAO 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cerebral blood flow changes after mild head trauma imaging with SPECT HMPAO .
	manualset3
138163	1	407216	5	NULL	NULL	0	NULL	one-dish meal 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A one-dish meal , Chinese noodle , became positive with an appropriate concentration of NaCl plus a MSG-5 ` ribonucleotide mixture , but not with NaCl alone .
	manualset3
138164	2	407216	5	NULL	NULL	0	NULL	Chinese noodle 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A one-dish meal , Chinese noodle , became positive with an appropriate concentration of NaCl plus a MSG-5 ` ribonucleotide mixture , but not with NaCl alone .
	manualset3
138165	3	407216	5	NULL	NULL	0	NULL	appropriate concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A one-dish meal , Chinese noodle , became positive with an appropriate concentration of NaCl plus a MSG-5 ` ribonucleotide mixture , but not with NaCl alone .
	manualset3
138166	4	407216	5	NULL	NULL	0	NULL	NaCl plus a MSG-5 ` ribonucleotide mixture	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A one-dish meal , Chinese noodle , became positive with an appropriate concentration of NaCl plus a MSG-5 ` ribonucleotide mixture , but not with NaCl alone .
	manualset3
138167	5	407216	5	NULL	NULL	0	NULL	NaCl 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A one-dish meal , Chinese noodle , became positive with an appropriate concentration of NaCl plus a MSG-5 ` ribonucleotide mixture , but not with NaCl alone .
	manualset3
138168	1	407217	5	NULL	NULL	0	NULL	Sodium iodide density gradients 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium iodide density gradients for the preparative buoyant density separations of DNA mixtures .
	manualset3
138169	2	407217	5	NULL	NULL	0	NULL	buoyant density separations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium iodide density gradients for the preparative buoyant density separations of DNA mixtures .
	manualset3
138170	3	407217	5	NULL	NULL	0	NULL	DNA mixtures	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium iodide density gradients for the preparative buoyant density separations of DNA mixtures .
	manualset3
138171	1	407218	5	NULL	NULL	0	NULL	Sodium nitroprusside	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium nitroprusside ( 10 ( -4 ) M ) induced a reproducible and endothelium-independent vasorelaxation .
	manualset3
138172	2	407218	5	NULL	NULL	0	NULL	( 10 ( -4 ) M )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium nitroprusside ( 10 ( -4 ) M ) induced a reproducible and endothelium-independent vasorelaxation .
	manualset3
138173	3	407218	5	NULL	NULL	0	NULL	endothelium-independent vasorelaxation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium nitroprusside ( 10 ( -4 ) M ) induced a reproducible and endothelium-independent vasorelaxation .
	manualset3
138174	1	407219	5	NULL	NULL	NULL	NULL	Sodium efflux ATPase	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Sodium or potassium efflux ATPase a fungal , bryophyte , and protozoal ATPase .
	manualset3
138175	2	407219	5	NULL	NULL	0	NULL	potassium efflux ATPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium or potassium efflux ATPase a fungal , bryophyte , and protozoal ATPase .
	manualset3
138176	3	407219	5	NULL	NULL	NULL	NULL	fungal ATPase 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Sodium or potassium efflux ATPase a fungal , bryophyte , and protozoal ATPase .
	manualset3
138177	4	407219	5	NULL	NULL	0	NULL	bryophyte ATPase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium or potassium efflux ATPase a fungal , bryophyte , and protozoal ATPase .
	manualset3
138178	5	407219	5	NULL	NULL	0	NULL	protozoal ATPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium or potassium efflux ATPase a fungal , bryophyte , and protozoal ATPase .
	manualset3
138179	1	407220	5	NULL	NULL	0	NULL	Sodium salicylate	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium salicylate inhibits the degradation of IkappaB , thus , NF-kappaB activation can not occur .
	manualset3
138180	2	407220	5	NULL	NULL	0	NULL	degradation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium salicylate inhibits the degradation of IkappaB , thus , NF-kappaB activation can not occur .
	manualset3
138181	3	407220	5	NULL	NULL	0	NULL	IkappaB 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium salicylate inhibits the degradation of IkappaB , thus , NF-kappaB activation can not occur .
	manualset3
138182	4	407220	5	NULL	NULL	0	NULL	NF-kappaB activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium salicylate inhibits the degradation of IkappaB , thus , NF-kappaB activation can not occur .
	manualset3
138183	1	407221	5	NULL	NULL	0	NULL	Sodium salicylate 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium salicylate is also a specific antagonist of 5-hydroxytryptamine , but its action is indirect , occurring only when the general serum level was raised above 10 or 20 mg .
	manualset3
138184	2	407221	5	NULL	NULL	0	NULL	specific antagonist of 5-hydroxytryptamine	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium salicylate is also a specific antagonist of 5-hydroxytryptamine , but its action is indirect , occurring only when the general serum level was raised above 10 or 20 mg .
	manualset3
138185	3	407221	5	NULL	NULL	0	NULL	general serum level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium salicylate is also a specific antagonist of 5-hydroxytryptamine , but its action is indirect , occurring only when the general serum level was raised above 10 or 20 mg .
	manualset3
138186	4	407221	5	NULL	NULL	0	NULL	10 or 20 mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium salicylate is also a specific antagonist of 5-hydroxytryptamine , but its action is indirect , occurring only when the general serum level was raised above 10 or 20 mg .
	manualset3
138187	1	407222	5	NULL	NULL	0	NULL	Soil pore water soluble Cd	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Soil pore water soluble Cd and free Cd2 + increased linearly with increasing total soil Cd ( R2 = 0.82 and 0.84 , respectively ; P & lt ; 0.001 ) .
	manualset3
138188	2	407222	5	NULL	NULL	0	NULL	free Cd2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Soil pore water soluble Cd and free Cd2 + increased linearly with increasing total soil Cd ( R2 = 0.82 and 0.84 , respectively ; P & lt ; 0.001 ) .
	manualset3
138189	3	407222	5	NULL	NULL	0	NULL	 total soil Cd	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Soil pore water soluble Cd and free Cd2 + increased linearly with increasing total soil Cd ( R2 = 0.82 and 0.84 , respectively ; P & lt ; 0.001 ) .
	manualset3
138190	4	407222	5	NULL	NULL	0	NULL	 R2 = 0.82 and 0.84 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Soil pore water soluble Cd and free Cd2 + increased linearly with increasing total soil Cd ( R2 = 0.82 and 0.84 , respectively ; P & lt ; 0.001 ) .
	manualset3
138191	5	407222	5	NULL	NULL	0	NULL	P & lt ; 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Soil pore water soluble Cd and free Cd2 + increased linearly with increasing total soil Cd ( R2 = 0.82 and 0.84 , respectively ; P & lt ; 0.001 ) .
	manualset3
138192	1	407223	5	NULL	NULL	0	NULL	Soil washing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Soil washing is one of the few permanent treatment alternatives to remove metal contaminants from soils .
	manualset3
138193	2	407223	5	NULL	NULL	0	NULL	one of the few 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Soil washing is one of the few permanent treatment alternatives to remove metal contaminants from soils .
	manualset3
138194	3	407223	5	NULL	NULL	0	NULL	permanent treatment alternatives	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Soil washing is one of the few permanent treatment alternatives to remove metal contaminants from soils .
	manualset3
138195	4	407223	5	NULL	NULL	0	NULL	metal contaminants	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Soil washing is one of the few permanent treatment alternatives to remove metal contaminants from soils .
	manualset3
138196	5	407223	5	NULL	NULL	0	NULL	soils 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Soil washing is one of the few permanent treatment alternatives to remove metal contaminants from soils .
	manualset3
138197	1	407224	5	NULL	NULL	0	NULL	Soleus muscles 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Soleus muscles of TRalpha1 - / - beta - / - mice showed increased contraction and relaxation times and the force-frequency relationship was shifted to the left .
	manualset3
138198	2	407224	5	NULL	NULL	0	NULL	TRalpha1 - / - beta - / - mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Soleus muscles of TRalpha1 - / - beta - / - mice showed increased contraction and relaxation times and the force-frequency relationship was shifted to the left .
	manualset3
138199	3	407224	5	NULL	NULL	NULL	NULL	contraction time	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Soleus muscles of TRalpha1 - / - beta - / - mice showed increased contraction and relaxation times and the force-frequency relationship was shifted to the left .
	manualset3
138200	4	407224	5	NULL	NULL	0	NULL	relaxation time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Soleus muscles of TRalpha1 - / - beta - / - mice showed increased contraction and relaxation times and the force-frequency relationship was shifted to the left .
	manualset3
138201	5	407224	5	NULL	NULL	0	NULL	force-frequency relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Soleus muscles of TRalpha1 - / - beta - / - mice showed increased contraction and relaxation times and the force-frequency relationship was shifted to the left .
	manualset3
138202	6	407224	5	NULL	NULL	0	NULL	left 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Soleus muscles of TRalpha1 - / - beta - / - mice showed increased contraction and relaxation times and the force-frequency relationship was shifted to the left .
	manualset3
138203	1	407225	5	NULL	NULL	NULL	NULL	Solid-phase extraction combined with dispersive liquid-liquid microextraction ( SPE-DLLME )	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Solid-phase extraction combined with dispersive liquid-liquid microextraction ( SPE-DLLME ) was applied for the extraction of six organophosphorous pesticides ( OPPs ) in water samples .
	manualset3
138204	2	407225	5	NULL	NULL	0	NULL	extraction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Solid-phase extraction combined with dispersive liquid-liquid microextraction ( SPE-DLLME ) was applied for the extraction of six organophosphorous pesticides ( OPPs ) in water samples .
	manualset3
138205	3	407225	5	NULL	NULL	0	NULL	six 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Solid-phase extraction combined with dispersive liquid-liquid microextraction ( SPE-DLLME ) was applied for the extraction of six organophosphorous pesticides ( OPPs ) in water samples .
	manualset3
138206	4	407225	5	NULL	NULL	0	NULL	organophosphorous pesticides ( OPPs )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Solid-phase extraction combined with dispersive liquid-liquid microextraction ( SPE-DLLME ) was applied for the extraction of six organophosphorous pesticides ( OPPs ) in water samples .
	manualset3
138207	5	407225	5	NULL	NULL	0	NULL	water samples	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Solid-phase extraction combined with dispersive liquid-liquid microextraction ( SPE-DLLME ) was applied for the extraction of six organophosphorous pesticides ( OPPs ) in water samples .
	manualset3
138208	1	407226	5	NULL	NULL	0	NULL	 p38 mitogen-activated protein kinase inhibitor , SB203580	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A p38 mitogen-activated protein kinase inhibitor , SB203580 , also inhibited the increase in IL-6 messenger RNA levels .
	manualset3
138209	2	407226	5	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A p38 mitogen-activated protein kinase inhibitor , SB203580 , also inhibited the increase in IL-6 messenger RNA levels .
	manualset3
138210	3	407226	5	NULL	NULL	0	NULL	IL-6 messenger RNA levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A p38 mitogen-activated protein kinase inhibitor , SB203580 , also inhibited the increase in IL-6 messenger RNA levels .
	manualset3
138211	1	407227	5	NULL	NULL	0	NULL	Solid-phase microextraction ( SPME )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Solid-phase microextraction ( SPME ) coupled with gas chromatography-mass spectrometry ( GC-MS ) was used to determine pesticide residues in Chinese herbal formulations .
	manualset3
138212	2	407227	5	NULL	NULL	0	NULL	gas chromatography-mass spectrometry ( GC-MS ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Solid-phase microextraction ( SPME ) coupled with gas chromatography-mass spectrometry ( GC-MS ) was used to determine pesticide residues in Chinese herbal formulations .
	manualset3
138213	3	407227	5	NULL	NULL	0	NULL	pesticide residues 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Solid-phase microextraction ( SPME ) coupled with gas chromatography-mass spectrometry ( GC-MS ) was used to determine pesticide residues in Chinese herbal formulations .
	manualset3
138214	4	407227	5	NULL	NULL	0	NULL	Chinese herbal formulations	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Solid-phase microextraction ( SPME ) coupled with gas chromatography-mass spectrometry ( GC-MS ) was used to determine pesticide residues in Chinese herbal formulations .
	manualset3
138215	1	407228	5	NULL	NULL	0	NULL	Solid organ transplants	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Solid organ transplants , corrective surgery for congenital malformations , improved cytostatic regimes for children with cancer , and respiratory care for premature infants are but a few examples of the changing face of medical practice .
	manualset3
138216	2	407228	5	NULL	NULL	0	NULL	corrective surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Solid organ transplants , corrective surgery for congenital malformations , improved cytostatic regimes for children with cancer , and respiratory care for premature infants are but a few examples of the changing face of medical practice .
	manualset3
138217	3	407228	5	NULL	NULL	0	NULL	congenital malformations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Solid organ transplants , corrective surgery for congenital malformations , improved cytostatic regimes for children with cancer , and respiratory care for premature infants are but a few examples of the changing face of medical practice .
	manualset3
138218	4	407228	5	NULL	NULL	0	NULL	cytostatic regimes	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Solid organ transplants , corrective surgery for congenital malformations , improved cytostatic regimes for children with cancer , and respiratory care for premature infants are but a few examples of the changing face of medical practice .
	manualset3
138219	5	407228	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Solid organ transplants , corrective surgery for congenital malformations , improved cytostatic regimes for children with cancer , and respiratory care for premature infants are but a few examples of the changing face of medical practice .
	manualset3
138220	6	407228	5	NULL	NULL	0	NULL	cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Solid organ transplants , corrective surgery for congenital malformations , improved cytostatic regimes for children with cancer , and respiratory care for premature infants are but a few examples of the changing face of medical practice .
	manualset3
138221	7	407228	5	NULL	NULL	0	NULL	respiratory care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Solid organ transplants , corrective surgery for congenital malformations , improved cytostatic regimes for children with cancer , and respiratory care for premature infants are but a few examples of the changing face of medical practice .
	manualset3
138222	8	407228	5	NULL	NULL	0	NULL	premature infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Solid organ transplants , corrective surgery for congenital malformations , improved cytostatic regimes for children with cancer , and respiratory care for premature infants are but a few examples of the changing face of medical practice .
	manualset3
138223	9	407228	5	NULL	NULL	0	NULL	few examples	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Solid organ transplants , corrective surgery for congenital malformations , improved cytostatic regimes for children with cancer , and respiratory care for premature infants are but a few examples of the changing face of medical practice .
	manualset3
138224	10	407228	5	NULL	NULL	0	NULL	changing face 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Solid organ transplants , corrective surgery for congenital malformations , improved cytostatic regimes for children with cancer , and respiratory care for premature infants are but a few examples of the changing face of medical practice .
	manualset3
138225	11	407228	5	NULL	NULL	0	NULL	medical practice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Solid organ transplants , corrective surgery for congenital malformations , improved cytostatic regimes for children with cancer , and respiratory care for premature infants are but a few examples of the changing face of medical practice .
	manualset3
138226	1	407229	5	NULL	NULL	0	NULL	Solid phase DNA extraction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Solid phase DNA extraction on PDMS and direct amplification .
	manualset3
138227	2	407229	5	NULL	NULL	0	NULL	PDMS 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Solid phase DNA extraction on PDMS and direct amplification .
	manualset3
138228	3	407229	5	NULL	NULL	0	NULL	direct amplification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Solid phase DNA extraction on PDMS and direct amplification .
	manualset3
138229	1	407230	5	NULL	NULL	0	NULL	Solid tumor nests	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Solid tumor nests were surrounded by dense IgG4-positive plasma cells and fibrosis at both the primary site and metastatic lymph nodes .
	manualset3
138230	2	407230	5	NULL	NULL	0	NULL	dense IgG4-positive plasma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Solid tumor nests were surrounded by dense IgG4-positive plasma cells and fibrosis at both the primary site and metastatic lymph nodes .
	manualset3
138231	3	407230	5	NULL	NULL	0	NULL	fibrosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Solid tumor nests were surrounded by dense IgG4-positive plasma cells and fibrosis at both the primary site and metastatic lymph nodes .
	manualset3
138232	4	407230	5	NULL	NULL	0	NULL	primary site	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Solid tumor nests were surrounded by dense IgG4-positive plasma cells and fibrosis at both the primary site and metastatic lymph nodes .
	manualset3
138233	5	407230	5	NULL	NULL	0	NULL	metastatic lymph nodes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Solid tumor nests were surrounded by dense IgG4-positive plasma cells and fibrosis at both the primary site and metastatic lymph nodes .
	manualset3
138444	1	407231	5	NULL	NULL	0	NULL	Solitary plasmocytoma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Solitary plasmocytoma : improvement in critical organs sparing by means of helical tomotherapy .
	manualset3
138445	2	407231	5	NULL	NULL	0	NULL	improvement 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Solitary plasmocytoma : improvement in critical organs sparing by means of helical tomotherapy .
	manualset3
138446	3	407231	5	NULL	NULL	0	NULL	critical organs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Solitary plasmocytoma : improvement in critical organs sparing by means of helical tomotherapy .
	manualset3
138447	4	407231	5	NULL	NULL	0	NULL	helical tomotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Solitary plasmocytoma : improvement in critical organs sparing by means of helical tomotherapy .
	manualset3
138448	1	407232	5	NULL	NULL	0	NULL	Solitary vertebral plasmacytoma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Solitary vertebral plasmacytoma causing compression fracture in a patient with multiple vertebral hemangiomas : a diagnosis easily missed !
	manualset3
138449	2	407232	5	NULL	NULL	0	NULL	compression fracture	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Solitary vertebral plasmacytoma causing compression fracture in a patient with multiple vertebral hemangiomas : a diagnosis easily missed !
	manualset3
138450	3	407232	5	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Solitary vertebral plasmacytoma causing compression fracture in a patient with multiple vertebral hemangiomas : a diagnosis easily missed !
	manualset3
138451	4	407232	5	NULL	NULL	0	NULL	multiple vertebral hemangiomas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Solitary vertebral plasmacytoma causing compression fracture in a patient with multiple vertebral hemangiomas : a diagnosis easily missed !
	manualset3
138452	5	407232	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Solitary vertebral plasmacytoma causing compression fracture in a patient with multiple vertebral hemangiomas : a diagnosis easily missed !
	manualset3
138453	1	407233	5	NULL	NULL	0	NULL	Solubility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Solubility of DCF was increased by the addition of M-beta-CD .
	manualset3
138454	2	407233	5	NULL	NULL	0	NULL	DCF 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Solubility of DCF was increased by the addition of M-beta-CD .
	manualset3
138455	3	407233	5	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Solubility of DCF was increased by the addition of M-beta-CD .
	manualset3
138456	4	407233	5	NULL	NULL	0	NULL	M-beta-CD	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Solubility of DCF was increased by the addition of M-beta-CD .
	manualset3
138457	1	407234	5	NULL	NULL	0	NULL	Solubilization 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Solubilization of bound lactate dehydrogenase by NADH in homogenates of trout skeletal muscle as a function of tissue concentration .
	manualset3
138458	2	407234	5	NULL	NULL	0	NULL	bound lactate dehydrogenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Solubilization of bound lactate dehydrogenase by NADH in homogenates of trout skeletal muscle as a function of tissue concentration .
	manualset3
138459	3	407234	5	NULL	NULL	0	NULL	NADH 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Solubilization of bound lactate dehydrogenase by NADH in homogenates of trout skeletal muscle as a function of tissue concentration .
	manualset3
138460	4	407234	5	NULL	NULL	0	NULL	homogenates 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Solubilization of bound lactate dehydrogenase by NADH in homogenates of trout skeletal muscle as a function of tissue concentration .
	manualset3
138461	5	407234	5	NULL	NULL	0	NULL	trout skeletal muscle	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Solubilization of bound lactate dehydrogenase by NADH in homogenates of trout skeletal muscle as a function of tissue concentration .
	manualset3
138462	6	407234	5	NULL	NULL	NULL	NULL	function 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Solubilization of bound lactate dehydrogenase by NADH in homogenates of trout skeletal muscle as a function of tissue concentration .
	manualset3
138463	7	407234	5	NULL	NULL	0	NULL	tissue concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Solubilization of bound lactate dehydrogenase by NADH in homogenates of trout skeletal muscle as a function of tissue concentration .
	manualset3
138464	1	407235	5	NULL	NULL	0	NULL	Soluble-insoluble self-oscillation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Soluble-insoluble self-oscillation of the polymer was first achieved without adding an oxidizing agent .
	manualset3
138465	2	407235	5	NULL	NULL	0	NULL	polymer 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Soluble-insoluble self-oscillation of the polymer was first achieved without adding an oxidizing agent .
	manualset3
138466	3	407235	5	NULL	NULL	0	NULL	oxidizing agent 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Soluble-insoluble self-oscillation of the polymer was first achieved without adding an oxidizing agent .
	manualset3
138467	1	407236	5	NULL	NULL	0	NULL	pamphlet 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A pamphlet in Spanish , featuring a picture of an elderly Latina listening to the phone message , describes how to access the tape .
	manualset3
138468	2	407236	5	NULL	NULL	0	NULL	Spanish 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A pamphlet in Spanish , featuring a picture of an elderly Latina listening to the phone message , describes how to access the tape .
	manualset3
138469	3	407236	5	NULL	NULL	0	NULL	picture 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A pamphlet in Spanish , featuring a picture of an elderly Latina listening to the phone message , describes how to access the tape .
	manualset3
138470	4	407236	5	NULL	NULL	0	NULL	elderly Latina 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A pamphlet in Spanish , featuring a picture of an elderly Latina listening to the phone message , describes how to access the tape .
	manualset3
138471	5	407236	5	NULL	NULL	0	NULL	phone message 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A pamphlet in Spanish , featuring a picture of an elderly Latina listening to the phone message , describes how to access the tape .
	manualset3
138472	6	407236	5	NULL	NULL	0	NULL	tape 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A pamphlet in Spanish , featuring a picture of an elderly Latina listening to the phone message , describes how to access the tape .
	manualset3
138473	1	407237	5	NULL	NULL	0	NULL	high-load ring-opening metathesis polymerization ( ROMP ) - derived oligomeric triazole phosphates ( OTP ) 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Soluble , high-load ring-opening metathesis polymerization ( ROMP ) - derived oligomeric triazole phosphates ( OTP ) are reported for application as efficient triazolating reagents of nucleophilic species .
	manualset3
138474	2	407237	5	NULL	NULL	0	NULL	application 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Soluble , high-load ring-opening metathesis polymerization ( ROMP ) - derived oligomeric triazole phosphates ( OTP ) are reported for application as efficient triazolating reagents of nucleophilic species .
	manualset3
138475	3	407237	5	NULL	NULL	0	NULL	efficient triazolating reagents 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Soluble , high-load ring-opening metathesis polymerization ( ROMP ) - derived oligomeric triazole phosphates ( OTP ) are reported for application as efficient triazolating reagents of nucleophilic species .
	manualset3
138476	4	407237	5	NULL	NULL	0	NULL	nucleophilic species	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Soluble , high-load ring-opening metathesis polymerization ( ROMP ) - derived oligomeric triazole phosphates ( OTP ) are reported for application as efficient triazolating reagents of nucleophilic species .
	manualset3
138477	1	407238	5	NULL	NULL	0	NULL	guanylate cyclase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Soluble guanylate cyclase is an enzyme that catalyzes formation of cGMP from GTP and is a member of the nucleotide cyclase family of enzymes .
	manualset3
138478	2	407238	5	NULL	NULL	0	NULL	enzyme 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Soluble guanylate cyclase is an enzyme that catalyzes formation of cGMP from GTP and is a member of the nucleotide cyclase family of enzymes .
	manualset3
138479	3	407238	5	NULL	NULL	0	NULL	formation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Soluble guanylate cyclase is an enzyme that catalyzes formation of cGMP from GTP and is a member of the nucleotide cyclase family of enzymes .
	manualset3
138480	4	407238	5	NULL	NULL	0	NULL	cGMP 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Soluble guanylate cyclase is an enzyme that catalyzes formation of cGMP from GTP and is a member of the nucleotide cyclase family of enzymes .
	manualset3
138481	5	407238	5	NULL	NULL	0	NULL	GTP 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Soluble guanylate cyclase is an enzyme that catalyzes formation of cGMP from GTP and is a member of the nucleotide cyclase family of enzymes .
	manualset3
138482	6	407238	5	NULL	NULL	0	NULL	member 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Soluble guanylate cyclase is an enzyme that catalyzes formation of cGMP from GTP and is a member of the nucleotide cyclase family of enzymes .
	manualset3
138483	7	407238	5	NULL	NULL	0	NULL	nucleotide cyclase family of enzymes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Soluble guanylate cyclase is an enzyme that catalyzes formation of cGMP from GTP and is a member of the nucleotide cyclase family of enzymes .
	manualset3
138484	1	407239	5	NULL	NULL	0	NULL	Soluble solids ( SS )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Soluble solids ( SS ) , titratable acidity ( TA ) , levels of sugars ( saccharose , fructose , and glucose ) , and organic acids ( citric and malic acids ) were also determined .
	manualset3
138485	2	407239	5	NULL	NULL	0	NULL	titratable acidity ( TA )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Soluble solids ( SS ) , titratable acidity ( TA ) , levels of sugars ( saccharose , fructose , and glucose ) , and organic acids ( citric and malic acids ) were also determined .
	manualset3
138486	3	407239	5	NULL	NULL	0	NULL	levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Soluble solids ( SS ) , titratable acidity ( TA ) , levels of sugars ( saccharose , fructose , and glucose ) , and organic acids ( citric and malic acids ) were also determined .
	manualset3
138487	4	407239	5	NULL	NULL	0	NULL	sugars 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Soluble solids ( SS ) , titratable acidity ( TA ) , levels of sugars ( saccharose , fructose , and glucose ) , and organic acids ( citric and malic acids ) were also determined .
	manualset3
138488	5	407239	5	NULL	NULL	0	NULL	saccharose 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Soluble solids ( SS ) , titratable acidity ( TA ) , levels of sugars ( saccharose , fructose , and glucose ) , and organic acids ( citric and malic acids ) were also determined .
	manualset3
138489	6	407239	5	NULL	NULL	0	NULL	fructose 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Soluble solids ( SS ) , titratable acidity ( TA ) , levels of sugars ( saccharose , fructose , and glucose ) , and organic acids ( citric and malic acids ) were also determined .
	manualset3
138490	7	407239	5	NULL	NULL	0	NULL	glucose 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Soluble solids ( SS ) , titratable acidity ( TA ) , levels of sugars ( saccharose , fructose , and glucose ) , and organic acids ( citric and malic acids ) were also determined .
	manualset3
138491	8	407239	5	NULL	NULL	0	NULL	organic acids	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Soluble solids ( SS ) , titratable acidity ( TA ) , levels of sugars ( saccharose , fructose , and glucose ) , and organic acids ( citric and malic acids ) were also determined .
	manualset3
138492	9	407239	5	NULL	NULL	0	NULL	citric acid	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Soluble solids ( SS ) , titratable acidity ( TA ) , levels of sugars ( saccharose , fructose , and glucose ) , and organic acids ( citric and malic acids ) were also determined .
	manualset3
138493	10	407239	5	NULL	NULL	0	NULL	malic acids	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Soluble solids ( SS ) , titratable acidity ( TA ) , levels of sugars ( saccharose , fructose , and glucose ) , and organic acids ( citric and malic acids ) were also determined .
	manualset3
138494	1	407240	5	NULL	NULL	0	NULL	Solution-phase incubation experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Solution-phase incubation experiments have shown that , although IPNS can turn over analogs with a diverse range of hydrocarbon side chains in the third ( valinyl ) position of its substrate , the enzyme is much less tolerant of polar residues in this position .
	manualset3
138495	2	407240	5	NULL	NULL	NULL	NULL	IPNS 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Solution-phase incubation experiments have shown that , although IPNS can turn over analogs with a diverse range of hydrocarbon side chains in the third ( valinyl ) position of its substrate , the enzyme is much less tolerant of polar residues in this position .
	manualset3
138496	3	407240	5	NULL	NULL	0	NULL	analogs 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Solution-phase incubation experiments have shown that , although IPNS can turn over analogs with a diverse range of hydrocarbon side chains in the third ( valinyl ) position of its substrate , the enzyme is much less tolerant of polar residues in this position .
	manualset3
138497	4	407240	5	NULL	NULL	0	NULL	diverse range 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Solution-phase incubation experiments have shown that , although IPNS can turn over analogs with a diverse range of hydrocarbon side chains in the third ( valinyl ) position of its substrate , the enzyme is much less tolerant of polar residues in this position .
	manualset3
138498	5	407240	5	NULL	NULL	0	NULL	hydrocarbon side chains	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Solution-phase incubation experiments have shown that , although IPNS can turn over analogs with a diverse range of hydrocarbon side chains in the third ( valinyl ) position of its substrate , the enzyme is much less tolerant of polar residues in this position .
	manualset3
138499	6	407240	5	NULL	NULL	NULL	NULL	third ( valinyl ) position	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Solution-phase incubation experiments have shown that , although IPNS can turn over analogs with a diverse range of hydrocarbon side chains in the third ( valinyl ) position of its substrate , the enzyme is much less tolerant of polar residues in this position .
	manualset3
138500	7	407240	5	NULL	NULL	0	NULL	substrate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Solution-phase incubation experiments have shown that , although IPNS can turn over analogs with a diverse range of hydrocarbon side chains in the third ( valinyl ) position of its substrate , the enzyme is much less tolerant of polar residues in this position .
	manualset3
138501	8	407240	5	NULL	NULL	0	NULL	enzyme 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Solution-phase incubation experiments have shown that , although IPNS can turn over analogs with a diverse range of hydrocarbon side chains in the third ( valinyl ) position of its substrate , the enzyme is much less tolerant of polar residues in this position .
	manualset3
138502	9	407240	5	NULL	NULL	0	NULL	polar residues	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Solution-phase incubation experiments have shown that , although IPNS can turn over analogs with a diverse range of hydrocarbon side chains in the third ( valinyl ) position of its substrate , the enzyme is much less tolerant of polar residues in this position .
	manualset3
138503	10	407240	5	NULL	NULL	0	NULL	position 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Solution-phase incubation experiments have shown that , although IPNS can turn over analogs with a diverse range of hydrocarbon side chains in the third ( valinyl ) position of its substrate , the enzyme is much less tolerant of polar residues in this position .
	manualset3
138504	1	407241	5	NULL	NULL	0	NULL	Solution NMR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Solution NMR of this toxin indicated a conformational heterogeneity with the existence of different conformers in solution , at slow and intermediate exchange rates relative to the NMR chemical shift time scale , similar to that reported for alpha-GI and alpha-MI .
	manualset3
138505	2	407241	5	NULL	NULL	0	NULL	toxin 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Solution NMR of this toxin indicated a conformational heterogeneity with the existence of different conformers in solution , at slow and intermediate exchange rates relative to the NMR chemical shift time scale , similar to that reported for alpha-GI and alpha-MI .
	manualset3
138506	3	407241	5	NULL	NULL	0	NULL	conformational heterogeneity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Solution NMR of this toxin indicated a conformational heterogeneity with the existence of different conformers in solution , at slow and intermediate exchange rates relative to the NMR chemical shift time scale , similar to that reported for alpha-GI and alpha-MI .
	manualset3
138507	4	407241	5	NULL	NULL	0	NULL	existence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Solution NMR of this toxin indicated a conformational heterogeneity with the existence of different conformers in solution , at slow and intermediate exchange rates relative to the NMR chemical shift time scale , similar to that reported for alpha-GI and alpha-MI .
	manualset3
138508	5	407241	5	NULL	NULL	0	NULL	different conformers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Solution NMR of this toxin indicated a conformational heterogeneity with the existence of different conformers in solution , at slow and intermediate exchange rates relative to the NMR chemical shift time scale , similar to that reported for alpha-GI and alpha-MI .
	manualset3
138509	6	407241	5	NULL	NULL	0	NULL	solution 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Solution NMR of this toxin indicated a conformational heterogeneity with the existence of different conformers in solution , at slow and intermediate exchange rates relative to the NMR chemical shift time scale , similar to that reported for alpha-GI and alpha-MI .
	manualset3
138510	7	407241	5	NULL	NULL	0	NULL	slow exchange rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Solution NMR of this toxin indicated a conformational heterogeneity with the existence of different conformers in solution , at slow and intermediate exchange rates relative to the NMR chemical shift time scale , similar to that reported for alpha-GI and alpha-MI .
	manualset3
138511	8	407241	5	NULL	NULL	0	NULL	intermediate exchange rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Solution NMR of this toxin indicated a conformational heterogeneity with the existence of different conformers in solution , at slow and intermediate exchange rates relative to the NMR chemical shift time scale , similar to that reported for alpha-GI and alpha-MI .
	manualset3
138512	9	407241	5	NULL	NULL	0	NULL	NMR chemical shift time scale	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Solution NMR of this toxin indicated a conformational heterogeneity with the existence of different conformers in solution , at slow and intermediate exchange rates relative to the NMR chemical shift time scale , similar to that reported for alpha-GI and alpha-MI .
	manualset3
138513	10	407241	5	NULL	NULL	0	NULL	alpha-GI	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Solution NMR of this toxin indicated a conformational heterogeneity with the existence of different conformers in solution , at slow and intermediate exchange rates relative to the NMR chemical shift time scale , similar to that reported for alpha-GI and alpha-MI .
	manualset3
138514	11	407241	5	NULL	NULL	0	NULL	alpha-MI	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Solution NMR of this toxin indicated a conformational heterogeneity with the existence of different conformers in solution , at slow and intermediate exchange rates relative to the NMR chemical shift time scale , similar to that reported for alpha-GI and alpha-MI .
	manualset3
138515	1	407242	5	NULL	NULL	0	NULL	problem 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Solving the problem at the source : Controlling Mn release at the sediment-water interface via hypolimnetic oxygenation .
	manualset3
138516	2	407242	5	NULL	NULL	0	NULL	source 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Solving the problem at the source : Controlling Mn release at the sediment-water interface via hypolimnetic oxygenation .
	manualset3
138517	3	407242	5	NULL	NULL	0	NULL	Mn release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Solving the problem at the source : Controlling Mn release at the sediment-water interface via hypolimnetic oxygenation .
	manualset3
138518	4	407242	5	NULL	NULL	0	NULL	sediment-water interface	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Solving the problem at the source : Controlling Mn release at the sediment-water interface via hypolimnetic oxygenation .
	manualset3
138519	5	407242	5	NULL	NULL	0	NULL	hypolimnetic oxygenation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Solving the problem at the source : Controlling Mn release at the sediment-water interface via hypolimnetic oxygenation .
	manualset3
138520	1	407243	5	NULL	NULL	0	NULL	Somaclonal variation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Somaclonal variation is manifested as cytological abnormalities , frequent qualitative and quantitative phenotypic mutation , sequence change , and gene activation and silencing .
	manualset3
138521	2	407243	5	NULL	NULL	0	NULL	cytological abnormalities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Somaclonal variation is manifested as cytological abnormalities , frequent qualitative and quantitative phenotypic mutation , sequence change , and gene activation and silencing .
	manualset3
138522	3	407243	5	NULL	NULL	0	NULL	qualitative phenotypic mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Somaclonal variation is manifested as cytological abnormalities , frequent qualitative and quantitative phenotypic mutation , sequence change , and gene activation and silencing .
	manualset3
138523	4	407243	5	NULL	NULL	0	NULL	quantitative phenotypic mutation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Somaclonal variation is manifested as cytological abnormalities , frequent qualitative and quantitative phenotypic mutation , sequence change , and gene activation and silencing .
	manualset3
138524	5	407243	5	NULL	NULL	0	NULL	sequence change	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Somaclonal variation is manifested as cytological abnormalities , frequent qualitative and quantitative phenotypic mutation , sequence change , and gene activation and silencing .
	manualset3
138525	6	407243	5	NULL	NULL	0	NULL	gene activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Somaclonal variation is manifested as cytological abnormalities , frequent qualitative and quantitative phenotypic mutation , sequence change , and gene activation and silencing .
	manualset3
138526	7	407243	5	NULL	NULL	0	NULL	gene silencing 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Somaclonal variation is manifested as cytological abnormalities , frequent qualitative and quantitative phenotypic mutation , sequence change , and gene activation and silencing .
	manualset3
138527	1	407244	5	NULL	NULL	0	NULL	Somali patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Somali patients with malaria also had marked hypergammaglobulinemia , however , only in the IgG class .
	manualset3
138528	2	407244	5	NULL	NULL	0	NULL	malaria 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Somali patients with malaria also had marked hypergammaglobulinemia , however , only in the IgG class .
	manualset3
138529	3	407244	5	NULL	NULL	0	NULL	hypergammaglobulinemia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Somali patients with malaria also had marked hypergammaglobulinemia , however , only in the IgG class .
	manualset3
138530	4	407244	5	NULL	NULL	0	NULL	IgG class	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Somali patients with malaria also had marked hypergammaglobulinemia , however , only in the IgG class .
	manualset3
138531	1	407245	5	NULL	NULL	0	NULL	Somatic defects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatic defects at five loci , WT1 , CTNNB1 , WTX , TP53 and the imprinted 11p15 region , are implicated in Wilms tumor , the commonest childhood kidney cancer .
	manualset3
138532	2	407245	5	NULL	NULL	0	NULL	five 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatic defects at five loci , WT1 , CTNNB1 , WTX , TP53 and the imprinted 11p15 region , are implicated in Wilms tumor , the commonest childhood kidney cancer .
	manualset3
138533	3	407245	5	NULL	NULL	0	NULL	loci 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatic defects at five loci , WT1 , CTNNB1 , WTX , TP53 and the imprinted 11p15 region , are implicated in Wilms tumor , the commonest childhood kidney cancer .
	manualset3
138534	4	407245	5	NULL	NULL	0	NULL	WT1 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatic defects at five loci , WT1 , CTNNB1 , WTX , TP53 and the imprinted 11p15 region , are implicated in Wilms tumor , the commonest childhood kidney cancer .
	manualset3
138535	5	407245	5	NULL	NULL	0	NULL	CTNNB1 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatic defects at five loci , WT1 , CTNNB1 , WTX , TP53 and the imprinted 11p15 region , are implicated in Wilms tumor , the commonest childhood kidney cancer .
	manualset3
138536	6	407245	5	NULL	NULL	0	NULL	WTX 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatic defects at five loci , WT1 , CTNNB1 , WTX , TP53 and the imprinted 11p15 region , are implicated in Wilms tumor , the commonest childhood kidney cancer .
	manualset3
138537	7	407245	5	NULL	NULL	0	NULL	TP53 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatic defects at five loci , WT1 , CTNNB1 , WTX , TP53 and the imprinted 11p15 region , are implicated in Wilms tumor , the commonest childhood kidney cancer .
	manualset3
138538	8	407245	5	NULL	NULL	0	NULL	imprinted 11p15 region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatic defects at five loci , WT1 , CTNNB1 , WTX , TP53 and the imprinted 11p15 region , are implicated in Wilms tumor , the commonest childhood kidney cancer .
	manualset3
138539	9	407245	5	NULL	NULL	0	NULL	Wilms tumor , the commonest childhood kidney cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatic defects at five loci , WT1 , CTNNB1 , WTX , TP53 and the imprinted 11p15 region , are implicated in Wilms tumor , the commonest childhood kidney cancer .
	manualset3
138540	1	407246	5	NULL	NULL	0	NULL	panel 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A panel of seven cases of bcr-Ph1 + acute leukemia ( three nonlymphocytic and four lymphocytic ) was investigated with these intron 1-derived probes .
	manualset3
138541	2	407246	5	NULL	NULL	0	NULL	seven cases 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A panel of seven cases of bcr-Ph1 + acute leukemia ( three nonlymphocytic and four lymphocytic ) was investigated with these intron 1-derived probes .
	manualset3
138542	3	407246	5	NULL	NULL	0	NULL	bcr-Ph1 + acute leukemia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A panel of seven cases of bcr-Ph1 + acute leukemia ( three nonlymphocytic and four lymphocytic ) was investigated with these intron 1-derived probes .
	manualset3
138543	4	407246	5	NULL	NULL	0	NULL	three nonlymphocytic	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A panel of seven cases of bcr-Ph1 + acute leukemia ( three nonlymphocytic and four lymphocytic ) was investigated with these intron 1-derived probes .
	manualset3
138544	5	407246	5	NULL	NULL	0	NULL	four lymphocytic 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A panel of seven cases of bcr-Ph1 + acute leukemia ( three nonlymphocytic and four lymphocytic ) was investigated with these intron 1-derived probes .
	manualset3
138545	6	407246	5	NULL	NULL	0	NULL	intron 1-derived probes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A panel of seven cases of bcr-Ph1 + acute leukemia ( three nonlymphocytic and four lymphocytic ) was investigated with these intron 1-derived probes .
	manualset3
138546	1	407247	5	NULL	NULL	0	NULL	Somatomedin 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatomedin , alpha 2-inhibitor and hypoglycemic stress .
	manualset3
138547	2	407247	5	NULL	NULL	0	NULL	alpha 2-inhibitor	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatomedin , alpha 2-inhibitor and hypoglycemic stress .
	manualset3
138548	3	407247	5	NULL	NULL	0	NULL	hypoglycemic stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatomedin , alpha 2-inhibitor and hypoglycemic stress .
	manualset3
138549	1	407248	5	NULL	NULL	0	NULL	Somatomedin C	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatomedin C was purified from a Cohn IV fraction of human plasma by acid release followed by dialysis , ultrafiltration , Sephadex G-50 chromatography , and isoelectric focusing between pH 7 to 11 .
	manualset3
138550	2	407248	5	NULL	NULL	0	NULL	Cohn IV fraction	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatomedin C was purified from a Cohn IV fraction of human plasma by acid release followed by dialysis , ultrafiltration , Sephadex G-50 chromatography , and isoelectric focusing between pH 7 to 11 .
	manualset3
138551	3	407248	5	NULL	NULL	0	NULL	human plasma	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatomedin C was purified from a Cohn IV fraction of human plasma by acid release followed by dialysis , ultrafiltration , Sephadex G-50 chromatography , and isoelectric focusing between pH 7 to 11 .
	manualset3
138552	4	407248	5	NULL	NULL	0	NULL	acid release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatomedin C was purified from a Cohn IV fraction of human plasma by acid release followed by dialysis , ultrafiltration , Sephadex G-50 chromatography , and isoelectric focusing between pH 7 to 11 .
	manualset3
138553	5	407248	5	NULL	NULL	0	NULL	dialysis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatomedin C was purified from a Cohn IV fraction of human plasma by acid release followed by dialysis , ultrafiltration , Sephadex G-50 chromatography , and isoelectric focusing between pH 7 to 11 .
	manualset3
138554	6	407248	5	NULL	NULL	0	NULL	ultrafiltration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatomedin C was purified from a Cohn IV fraction of human plasma by acid release followed by dialysis , ultrafiltration , Sephadex G-50 chromatography , and isoelectric focusing between pH 7 to 11 .
	manualset3
138555	7	407248	5	NULL	NULL	0	NULL	Sephadex G-50 chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatomedin C was purified from a Cohn IV fraction of human plasma by acid release followed by dialysis , ultrafiltration , Sephadex G-50 chromatography , and isoelectric focusing between pH 7 to 11 .
	manualset3
138556	8	407248	5	NULL	NULL	0	NULL	isoelectric focusing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatomedin C was purified from a Cohn IV fraction of human plasma by acid release followed by dialysis , ultrafiltration , Sephadex G-50 chromatography , and isoelectric focusing between pH 7 to 11 .
	manualset3
138557	9	407248	5	NULL	NULL	0	NULL	pH 7 to 11	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatomedin C was purified from a Cohn IV fraction of human plasma by acid release followed by dialysis , ultrafiltration , Sephadex G-50 chromatography , and isoelectric focusing between pH 7 to 11 .
	manualset3
138558	1	407249	5	NULL	NULL	0	NULL	Somatosensory cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatosensory cortex : a comparison of the response to noxious thermal , mechanical , and electrical stimuli using functional magnetic resonance imaging .
	manualset3
138559	2	407249	5	NULL	NULL	0	NULL	comparison 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatosensory cortex : a comparison of the response to noxious thermal , mechanical , and electrical stimuli using functional magnetic resonance imaging .
	manualset3
138560	3	407249	5	NULL	NULL	0	NULL	response 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatosensory cortex : a comparison of the response to noxious thermal , mechanical , and electrical stimuli using functional magnetic resonance imaging .
	manualset3
138561	4	407249	5	NULL	NULL	0	NULL	noxious thermal stimuli 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatosensory cortex : a comparison of the response to noxious thermal , mechanical , and electrical stimuli using functional magnetic resonance imaging .
	manualset3
138562	5	407249	5	NULL	NULL	0	NULL	mechanical stimuli 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatosensory cortex : a comparison of the response to noxious thermal , mechanical , and electrical stimuli using functional magnetic resonance imaging .
	manualset3
138563	6	407249	5	NULL	NULL	0	NULL	electrical stimuli 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatosensory cortex : a comparison of the response to noxious thermal , mechanical , and electrical stimuli using functional magnetic resonance imaging .
	manualset3
138564	7	407249	5	NULL	NULL	0	NULL	functional magnetic resonance imaging 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatosensory cortex : a comparison of the response to noxious thermal , mechanical , and electrical stimuli using functional magnetic resonance imaging .
	manualset3
138565	1	407250	5	NULL	NULL	0	NULL	Somatostatin analogs	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatostatin analogs have been the mainstay of symptomatic management of patients with neuroendocrine tumors ( NETs ) for two decades with the main mechanism of action being inhibition of peptide release .
	manualset3
138566	2	407250	5	NULL	NULL	0	NULL	mainstay 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatostatin analogs have been the mainstay of symptomatic management of patients with neuroendocrine tumors ( NETs ) for two decades with the main mechanism of action being inhibition of peptide release .
	manualset3
138567	3	407250	5	NULL	NULL	0	NULL	symptomatic management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatostatin analogs have been the mainstay of symptomatic management of patients with neuroendocrine tumors ( NETs ) for two decades with the main mechanism of action being inhibition of peptide release .
	manualset3
138568	4	407250	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatostatin analogs have been the mainstay of symptomatic management of patients with neuroendocrine tumors ( NETs ) for two decades with the main mechanism of action being inhibition of peptide release .
	manualset3
138569	5	407250	5	NULL	NULL	0	NULL	neuroendocrine tumors ( NETs )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatostatin analogs have been the mainstay of symptomatic management of patients with neuroendocrine tumors ( NETs ) for two decades with the main mechanism of action being inhibition of peptide release .
	manualset3
138570	6	407250	5	NULL	NULL	0	NULL	two decades	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatostatin analogs have been the mainstay of symptomatic management of patients with neuroendocrine tumors ( NETs ) for two decades with the main mechanism of action being inhibition of peptide release .
	manualset3
138571	7	407250	5	NULL	NULL	0	NULL	mechanism of action	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatostatin analogs have been the mainstay of symptomatic management of patients with neuroendocrine tumors ( NETs ) for two decades with the main mechanism of action being inhibition of peptide release .
	manualset3
138572	8	407250	5	NULL	NULL	NULL	NULL	inhibition 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Somatostatin analogs have been the mainstay of symptomatic management of patients with neuroendocrine tumors ( NETs ) for two decades with the main mechanism of action being inhibition of peptide release .
	manualset3
138573	9	407250	5	NULL	NULL	0	NULL	peptide release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatostatin analogs have been the mainstay of symptomatic management of patients with neuroendocrine tumors ( NETs ) for two decades with the main mechanism of action being inhibition of peptide release .
	manualset3
138574	1	407251	5	NULL	NULL	0	NULL	Somatostatin receptor expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatostatin receptor expression , tumor response , and quality of life in patients with advanced hepatocellular carcinoma treated with long-acting octreotide .
	manualset3
138575	2	407251	5	NULL	NULL	0	NULL	tumor response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatostatin receptor expression , tumor response , and quality of life in patients with advanced hepatocellular carcinoma treated with long-acting octreotide .
	manualset3
138576	3	407251	5	NULL	NULL	0	NULL	quality of life 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatostatin receptor expression , tumor response , and quality of life in patients with advanced hepatocellular carcinoma treated with long-acting octreotide .
	manualset3
138577	4	407251	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatostatin receptor expression , tumor response , and quality of life in patients with advanced hepatocellular carcinoma treated with long-acting octreotide .
	manualset3
138578	5	407251	5	NULL	NULL	0	NULL	advanced hepatocellular carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatostatin receptor expression , tumor response , and quality of life in patients with advanced hepatocellular carcinoma treated with long-acting octreotide .
	manualset3
138579	6	407251	5	NULL	NULL	0	NULL	octreotide 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Somatostatin receptor expression , tumor response , and quality of life in patients with advanced hepatocellular carcinoma treated with long-acting octreotide .
	manualset3
138580	1	407252	5	NULL	NULL	0	NULL	18 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Some 18 anopheline species are tentatively graded as having low , medium or high natural human blood indices .
	manualset3
138581	2	407252	5	NULL	NULL	0	NULL	anopheline species 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Some 18 anopheline species are tentatively graded as having low , medium or high natural human blood indices .
	manualset3
138582	3	407252	5	NULL	NULL	0	NULL	low , medium or high natural human blood indices	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some 18 anopheline species are tentatively graded as having low , medium or high natural human blood indices .
	manualset3
138583	1	407253	5	NULL	NULL	0	NULL	50 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Some 50 % of the decedents had alcohol or drugs present at the time of death ; among American Indians/Alaska Natives , 74 % had drugs or alcohol present ( p = .003 ) .
	manualset3
138584	2	407253	5	NULL	NULL	0	NULL	decedents 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Some 50 % of the decedents had alcohol or drugs present at the time of death ; among American Indians/Alaska Natives , 74 % had drugs or alcohol present ( p = .003 ) .
	manualset3
138585	3	407253	5	NULL	NULL	0	NULL	alcohol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Some 50 % of the decedents had alcohol or drugs present at the time of death ; among American Indians/Alaska Natives , 74 % had drugs or alcohol present ( p = .003 ) .
	manualset3
138586	4	407253	5	NULL	NULL	0	NULL	drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Some 50 % of the decedents had alcohol or drugs present at the time of death ; among American Indians/Alaska Natives , 74 % had drugs or alcohol present ( p = .003 ) .
	manualset3
138587	5	407253	5	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Some 50 % of the decedents had alcohol or drugs present at the time of death ; among American Indians/Alaska Natives , 74 % had drugs or alcohol present ( p = .003 ) .
	manualset3
138588	6	407253	5	NULL	NULL	0	NULL	death 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Some 50 % of the decedents had alcohol or drugs present at the time of death ; among American Indians/Alaska Natives , 74 % had drugs or alcohol present ( p = .003 ) .
	manualset3
138589	7	407253	5	NULL	NULL	0	NULL	American Indians/Alaska Natives	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Some 50 % of the decedents had alcohol or drugs present at the time of death ; among American Indians/Alaska Natives , 74 % had drugs or alcohol present ( p = .003 ) .
	manualset3
138590	8	407253	5	NULL	NULL	0	NULL	74 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Some 50 % of the decedents had alcohol or drugs present at the time of death ; among American Indians/Alaska Natives , 74 % had drugs or alcohol present ( p = .003 ) .
	manualset3
138591	9	407253	5	NULL	NULL	0	NULL	drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Some 50 % of the decedents had alcohol or drugs present at the time of death ; among American Indians/Alaska Natives , 74 % had drugs or alcohol present ( p = .003 ) .
	manualset3
138592	10	407253	5	NULL	NULL	0	NULL	alcohol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Some 50 % of the decedents had alcohol or drugs present at the time of death ; among American Indians/Alaska Natives , 74 % had drugs or alcohol present ( p = .003 ) .
	manualset3
138593	11	407253	5	NULL	NULL	0	NULL	 p = .003 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Some 50 % of the decedents had alcohol or drugs present at the time of death ; among American Indians/Alaska Natives , 74 % had drugs or alcohol present ( p = .003 ) .
	manualset3
138594	1	407254	5	NULL	NULL	0	NULL	adhesion molecules	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Some adhesion molecules , including ICAM-1 and VCAM-1 , exist in soluble , circulating forms that retain ligand-binding activity .
	manualset3
138595	2	407254	5	NULL	NULL	0	NULL	ICAM-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Some adhesion molecules , including ICAM-1 and VCAM-1 , exist in soluble , circulating forms that retain ligand-binding activity .
	manualset3
138596	3	407254	5	NULL	NULL	0	NULL	VCAM-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Some adhesion molecules , including ICAM-1 and VCAM-1 , exist in soluble , circulating forms that retain ligand-binding activity .
	manualset3
138597	4	407254	5	NULL	NULL	0	NULL	circulating forms	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Some adhesion molecules , including ICAM-1 and VCAM-1 , exist in soluble , circulating forms that retain ligand-binding activity .
	manualset3
138598	5	407254	5	NULL	NULL	0	NULL	ligand-binding activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Some adhesion molecules , including ICAM-1 and VCAM-1 , exist in soluble , circulating forms that retain ligand-binding activity .
	manualset3
138599	1	407255	5	NULL	NULL	0	NULL	allergic sheep 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Some allergic sheep respond to inhalation of Ascaris suum antigen with both immediate and late increases in airflow resistance ( late response ) .
	manualset3
138600	2	407255	5	NULL	NULL	0	NULL	inhalation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some allergic sheep respond to inhalation of Ascaris suum antigen with both immediate and late increases in airflow resistance ( late response ) .
	manualset3
138601	3	407255	5	NULL	NULL	0	NULL	Ascaris suum antigen	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Some allergic sheep respond to inhalation of Ascaris suum antigen with both immediate and late increases in airflow resistance ( late response ) .
	manualset3
138602	4	407255	5	NULL	NULL	0	NULL	airflow resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Some allergic sheep respond to inhalation of Ascaris suum antigen with both immediate and late increases in airflow resistance ( late response ) .
	manualset3
138603	5	407255	5	NULL	NULL	0	NULL	late response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Some allergic sheep respond to inhalation of Ascaris suum antigen with both immediate and late increases in airflow resistance ( late response ) .
	manualset3
138604	1	407256	5	NULL	NULL	0	NULL	parallel analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A parallel analysis with nonviolent offending as the dependent variable failed to find significant interactions .
	manualset3
138605	2	407256	5	NULL	NULL	0	NULL	dependent variable	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A parallel analysis with nonviolent offending as the dependent variable failed to find significant interactions .
	manualset3
138606	3	407256	5	NULL	NULL	0	NULL	interactions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A parallel analysis with nonviolent offending as the dependent variable failed to find significant interactions .
	manualset3
138607	1	407257	5	NULL	NULL	0	NULL	hospitals 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Some are particularly relevant to hospitals in the developed world , whereas others can apply to all hospitals .
	manualset3
138608	2	407257	5	NULL	NULL	0	NULL	developed world	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Some are particularly relevant to hospitals in the developed world , whereas others can apply to all hospitals .
	manualset3
138609	3	407257	5	NULL	NULL	0	NULL	hospitals 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Some are particularly relevant to hospitals in the developed world , whereas others can apply to all hospitals .
	manualset3
138610	1	407258	5	NULL	NULL	0	NULL	aspects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some aspects of ocular and neurological manifestations of the Groenblad-Strandberg syndrome .
	manualset3
138611	2	407258	5	NULL	NULL	0	NULL	ocular manifestations 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Some aspects of ocular and neurological manifestations of the Groenblad-Strandberg syndrome .
	manualset3
138612	3	407258	5	NULL	NULL	0	NULL	neurological manifestations 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Some aspects of ocular and neurological manifestations of the Groenblad-Strandberg syndrome .
	manualset3
138613	4	407258	5	NULL	NULL	0	NULL	Groenblad-Strandberg syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Some aspects of ocular and neurological manifestations of the Groenblad-Strandberg syndrome .
	manualset3
138614	1	407259	5	NULL	NULL	0	NULL	aspects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some aspects of the treatment of skin diseases .
	manualset3
138615	2	407259	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Some aspects of the treatment of skin diseases .
	manualset3
138616	3	407259	5	NULL	NULL	0	NULL	skin diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Some aspects of the treatment of skin diseases .
	manualset3
138617	1	407260	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Some authors discussed the possibility of postoperative radiotherapy although only six patients developed recurrence of their clinical features several years after operation and also the efficacy of such a procedure has not been proved .
	manualset3
138618	2	407260	5	NULL	NULL	0	NULL	possibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some authors discussed the possibility of postoperative radiotherapy although only six patients developed recurrence of their clinical features several years after operation and also the efficacy of such a procedure has not been proved .
	manualset3
138619	3	407260	5	NULL	NULL	0	NULL	postoperative radiotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Some authors discussed the possibility of postoperative radiotherapy although only six patients developed recurrence of their clinical features several years after operation and also the efficacy of such a procedure has not been proved .
	manualset3
138620	4	407260	5	NULL	NULL	0	NULL	six 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Some authors discussed the possibility of postoperative radiotherapy although only six patients developed recurrence of their clinical features several years after operation and also the efficacy of such a procedure has not been proved .
	manualset3
138621	5	407260	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Some authors discussed the possibility of postoperative radiotherapy although only six patients developed recurrence of their clinical features several years after operation and also the efficacy of such a procedure has not been proved .
	manualset3
138622	6	407260	5	NULL	NULL	0	NULL	recurrence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Some authors discussed the possibility of postoperative radiotherapy although only six patients developed recurrence of their clinical features several years after operation and also the efficacy of such a procedure has not been proved .
	manualset3
138623	7	407260	5	NULL	NULL	0	NULL	clinical features	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Some authors discussed the possibility of postoperative radiotherapy although only six patients developed recurrence of their clinical features several years after operation and also the efficacy of such a procedure has not been proved .
	manualset3
138624	8	407260	5	NULL	NULL	0	NULL	years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Some authors discussed the possibility of postoperative radiotherapy although only six patients developed recurrence of their clinical features several years after operation and also the efficacy of such a procedure has not been proved .
	manualset3
138625	9	407260	5	NULL	NULL	0	NULL	operation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Some authors discussed the possibility of postoperative radiotherapy although only six patients developed recurrence of their clinical features several years after operation and also the efficacy of such a procedure has not been proved .
	manualset3
138626	10	407260	5	NULL	NULL	0	NULL	efficacy 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some authors discussed the possibility of postoperative radiotherapy although only six patients developed recurrence of their clinical features several years after operation and also the efficacy of such a procedure has not been proved .
	manualset3
138627	11	407260	5	NULL	NULL	0	NULL	procedure 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Some authors discussed the possibility of postoperative radiotherapy although only six patients developed recurrence of their clinical features several years after operation and also the efficacy of such a procedure has not been proved .
	manualset3
138628	1	407261	5	NULL	NULL	0	NULL	clinical findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Some clinical findings in XLI , such as cryptorchidism in patients and delayed labor in their mothers , were important features for diagnosis .
	manualset3
138629	2	407261	5	NULL	NULL	0	NULL	XLI 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Some clinical findings in XLI , such as cryptorchidism in patients and delayed labor in their mothers , were important features for diagnosis .
	manualset3
138630	3	407261	5	NULL	NULL	0	NULL	cryptorchidism 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Some clinical findings in XLI , such as cryptorchidism in patients and delayed labor in their mothers , were important features for diagnosis .
	manualset3
138631	4	407261	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Some clinical findings in XLI , such as cryptorchidism in patients and delayed labor in their mothers , were important features for diagnosis .
	manualset3
138632	5	407261	5	NULL	NULL	0	NULL	delayed labor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Some clinical findings in XLI , such as cryptorchidism in patients and delayed labor in their mothers , were important features for diagnosis .
	manualset3
138633	6	407261	5	NULL	NULL	0	NULL	mothers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Some clinical findings in XLI , such as cryptorchidism in patients and delayed labor in their mothers , were important features for diagnosis .
	manualset3
138634	7	407261	5	NULL	NULL	0	NULL	important features 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Some clinical findings in XLI , such as cryptorchidism in patients and delayed labor in their mothers , were important features for diagnosis .
	manualset3
138635	8	407261	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Some clinical findings in XLI , such as cryptorchidism in patients and delayed labor in their mothers , were important features for diagnosis .
	manualset3
138636	1	407262	5	NULL	NULL	0	NULL	coagulase negative staphylococci ( CNS ) species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Some coagulase negative staphylococci ( CNS ) species play an important role in the fermentation of meat and milk products and are considered as food-grade .
	manualset3
138637	2	407262	5	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some coagulase negative staphylococci ( CNS ) species play an important role in the fermentation of meat and milk products and are considered as food-grade .
	manualset3
138638	3	407262	5	NULL	NULL	0	NULL	fermentation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Some coagulase negative staphylococci ( CNS ) species play an important role in the fermentation of meat and milk products and are considered as food-grade .
	manualset3
138639	4	407262	5	NULL	NULL	0	NULL	meat 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Some coagulase negative staphylococci ( CNS ) species play an important role in the fermentation of meat and milk products and are considered as food-grade .
	manualset3
138640	5	407262	5	NULL	NULL	0	NULL	milk products	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Some coagulase negative staphylococci ( CNS ) species play an important role in the fermentation of meat and milk products and are considered as food-grade .
	manualset3
138641	6	407262	5	NULL	NULL	NULL	NULL	food-grade	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Some coagulase negative staphylococci ( CNS ) species play an important role in the fermentation of meat and milk products and are considered as food-grade .
	manualset3
138642	1	407263	5	NULL	NULL	0	NULL	conditions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some conditions promoting the synthesis of PHB and PHB/V by natural , mutant , and recombinant producers are considered .
	manualset3
138643	2	407263	5	NULL	NULL	0	NULL	synthesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Some conditions promoting the synthesis of PHB and PHB/V by natural , mutant , and recombinant producers are considered .
	manualset3
138644	3	407263	5	NULL	NULL	0	NULL	PHB 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Some conditions promoting the synthesis of PHB and PHB/V by natural , mutant , and recombinant producers are considered .
	manualset3
138645	5	407263	5	NULL	NULL	NULL	NULL	natural , mutant , and recombinant producers	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Some conditions promoting the synthesis of PHB and PHB/V by natural , mutant , and recombinant producers are considered .
	manualset3
138646	4	407263	5	NULL	NULL	0	NULL	PHB/V	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Some conditions promoting the synthesis of PHB and PHB/V by natural , mutant , and recombinant producers are considered .
	manualset3
138647	1	407264	5	NULL	NULL	0	NULL	critics 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Some critics have challenged the economic argument based on distal outcomes such as increased employee longevity and less morbidity later in life .
	manualset3
138648	2	407264	5	NULL	NULL	0	NULL	economic argument	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some critics have challenged the economic argument based on distal outcomes such as increased employee longevity and less morbidity later in life .
	manualset3
138649	3	407264	5	NULL	NULL	0	NULL	distal outcomes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some critics have challenged the economic argument based on distal outcomes such as increased employee longevity and less morbidity later in life .
	manualset3
138650	4	407264	5	NULL	NULL	0	NULL	increased employee longevity 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some critics have challenged the economic argument based on distal outcomes such as increased employee longevity and less morbidity later in life .
	manualset3
138651	5	407264	5	NULL	NULL	0	NULL	less morbidity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some critics have challenged the economic argument based on distal outcomes such as increased employee longevity and less morbidity later in life .
	manualset3
138652	6	407264	5	NULL	NULL	0	NULL	life 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Some critics have challenged the economic argument based on distal outcomes such as increased employee longevity and less morbidity later in life .
	manualset3
138653	1	407265	5	NULL	NULL	0	NULL	paratracheal neck metastasis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A paratracheal neck metastasis also developed in the same patient in early adulthood .
	manualset3
138654	2	407265	5	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A paratracheal neck metastasis also developed in the same patient in early adulthood .
	manualset3
138655	3	407265	5	NULL	NULL	0	NULL	early adulthood	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A paratracheal neck metastasis also developed in the same patient in early adulthood .
	manualset3
138656	1	407266	5	NULL	NULL	0	NULL	general physiology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some details of the general physiology of intestinal fat absorption are discussed taking triglyceride absorption as an example .
	manualset3
138657	2	407266	5	NULL	NULL	NULL	NULL	intestinal fat absorption	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Some details of the general physiology of intestinal fat absorption are discussed taking triglyceride absorption as an example .
	manualset3
138658	3	407266	5	NULL	NULL	NULL	NULL	triglyceride absorption	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Some details of the general physiology of intestinal fat absorption are discussed taking triglyceride absorption as an example .
	manualset3
138659	1	407267	5	NULL	NULL	0	NULL	individual disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Some differences were found for individual disorders , mostly anxiety .
	manualset3
138660	2	407267	5	NULL	NULL	0	NULL	anxiety 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Some differences were found for individual disorders , mostly anxiety .
	manualset3
138661	1	407268	5	NULL	NULL	0	NULL	drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Some drugs can influence multiple neutrophil functions .
	manualset3
138662	2	407268	5	NULL	NULL	NULL	NULL	multiple neutrophil functions	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Some drugs can influence multiple neutrophil functions .
	manualset3
138663	1	407269	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some effects of dopamine transporter and receptor ligands on discriminative stimulus , physiologic , and directly observable indices of opioid withdrawal in rhesus monkeys .
	manualset3
138664	2	407269	5	NULL	NULL	0	NULL	dopamine transporter	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Some effects of dopamine transporter and receptor ligands on discriminative stimulus , physiologic , and directly observable indices of opioid withdrawal in rhesus monkeys .
	manualset3
138665	3	407269	5	NULL	NULL	0	NULL	receptor ligands 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Some effects of dopamine transporter and receptor ligands on discriminative stimulus , physiologic , and directly observable indices of opioid withdrawal in rhesus monkeys .
	manualset3
138666	4	407269	5	NULL	NULL	0	NULL	discriminative stimulus 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some effects of dopamine transporter and receptor ligands on discriminative stimulus , physiologic , and directly observable indices of opioid withdrawal in rhesus monkeys .
	manualset3
138667	5	407269	5	NULL	NULL	0	NULL	physiologic , and directly observable indices	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some effects of dopamine transporter and receptor ligands on discriminative stimulus , physiologic , and directly observable indices of opioid withdrawal in rhesus monkeys .
	manualset3
138668	6	407269	5	NULL	NULL	NULL	NULL	 opioid withdrawal 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Some effects of dopamine transporter and receptor ligands on discriminative stimulus , physiologic , and directly observable indices of opioid withdrawal in rhesus monkeys .
	manualset3
138669	7	407269	5	NULL	NULL	0	NULL	rhesus monkeys	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Some effects of dopamine transporter and receptor ligands on discriminative stimulus , physiologic , and directly observable indices of opioid withdrawal in rhesus monkeys .
	manualset3
138670	1	407270	5	NULL	NULL	0	NULL	endogenous metabolites	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Some endogenous metabolites , particularly unesterified fatty acids , bile acids , L-tryptophan and bilirubin which are formed both under physiological conditions and in pathological states of the organism , e.g. , in uremia can displace drugs from their areas of binding on albumin molecule .
	manualset3
138671	2	407270	5	NULL	NULL	0	NULL	unesterified fatty acids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Some endogenous metabolites , particularly unesterified fatty acids , bile acids , L-tryptophan and bilirubin which are formed both under physiological conditions and in pathological states of the organism , e.g. , in uremia can displace drugs from their areas of binding on albumin molecule .
	manualset3
138672	3	407270	5	NULL	NULL	0	NULL	bile acids 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Some endogenous metabolites , particularly unesterified fatty acids , bile acids , L-tryptophan and bilirubin which are formed both under physiological conditions and in pathological states of the organism , e.g. , in uremia can displace drugs from their areas of binding on albumin molecule .
	manualset3
138673	4	407270	5	NULL	NULL	0	NULL	L-tryptophan 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Some endogenous metabolites , particularly unesterified fatty acids , bile acids , L-tryptophan and bilirubin which are formed both under physiological conditions and in pathological states of the organism , e.g. , in uremia can displace drugs from their areas of binding on albumin molecule .
	manualset3
138674	5	407270	5	NULL	NULL	0	NULL	bilirubin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Some endogenous metabolites , particularly unesterified fatty acids , bile acids , L-tryptophan and bilirubin which are formed both under physiological conditions and in pathological states of the organism , e.g. , in uremia can displace drugs from their areas of binding on albumin molecule .
	manualset3
138675	6	407270	5	NULL	NULL	0	NULL	physiological conditions	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some endogenous metabolites , particularly unesterified fatty acids , bile acids , L-tryptophan and bilirubin which are formed both under physiological conditions and in pathological states of the organism , e.g. , in uremia can displace drugs from their areas of binding on albumin molecule .
	manualset3
138676	7	407270	5	NULL	NULL	0	NULL	pathological states	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Some endogenous metabolites , particularly unesterified fatty acids , bile acids , L-tryptophan and bilirubin which are formed both under physiological conditions and in pathological states of the organism , e.g. , in uremia can displace drugs from their areas of binding on albumin molecule .
	manualset3
138677	8	407270	5	NULL	NULL	0	NULL	organism 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Some endogenous metabolites , particularly unesterified fatty acids , bile acids , L-tryptophan and bilirubin which are formed both under physiological conditions and in pathological states of the organism , e.g. , in uremia can displace drugs from their areas of binding on albumin molecule .
	manualset3
138678	9	407270	5	NULL	NULL	0	NULL	uremia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Some endogenous metabolites , particularly unesterified fatty acids , bile acids , L-tryptophan and bilirubin which are formed both under physiological conditions and in pathological states of the organism , e.g. , in uremia can displace drugs from their areas of binding on albumin molecule .
	manualset3
138679	10	407270	5	NULL	NULL	0	NULL	drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Some endogenous metabolites , particularly unesterified fatty acids , bile acids , L-tryptophan and bilirubin which are formed both under physiological conditions and in pathological states of the organism , e.g. , in uremia can displace drugs from their areas of binding on albumin molecule .
	manualset3
138680	11	407270	5	NULL	NULL	0	NULL	areas 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some endogenous metabolites , particularly unesterified fatty acids , bile acids , L-tryptophan and bilirubin which are formed both under physiological conditions and in pathological states of the organism , e.g. , in uremia can displace drugs from their areas of binding on albumin molecule .
	manualset3
138681	12	407270	5	NULL	NULL	0	NULL	albumin molecule	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Some endogenous metabolites , particularly unesterified fatty acids , bile acids , L-tryptophan and bilirubin which are formed both under physiological conditions and in pathological states of the organism , e.g. , in uremia can displace drugs from their areas of binding on albumin molecule .
	manualset3
138682	1	407271	5	NULL	NULL	0	NULL	factors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some factors affecting the capacity and serviceability of the compounds such as the nature and graininess of the abrasive , the quantity of the compound added to the container at a time are investigated .
	manualset3
138683	2	407271	5	NULL	NULL	0	NULL	capacity 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some factors affecting the capacity and serviceability of the compounds such as the nature and graininess of the abrasive , the quantity of the compound added to the container at a time are investigated .
	manualset3
138684	3	407271	5	NULL	NULL	0	NULL	serviceability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some factors affecting the capacity and serviceability of the compounds such as the nature and graininess of the abrasive , the quantity of the compound added to the container at a time are investigated .
	manualset3
138685	4	407271	5	NULL	NULL	0	NULL	compounds 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Some factors affecting the capacity and serviceability of the compounds such as the nature and graininess of the abrasive , the quantity of the compound added to the container at a time are investigated .
	manualset3
138686	5	407271	5	NULL	NULL	0	NULL	nature 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some factors affecting the capacity and serviceability of the compounds such as the nature and graininess of the abrasive , the quantity of the compound added to the container at a time are investigated .
	manualset3
138687	6	407271	5	NULL	NULL	0	NULL	graininess 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some factors affecting the capacity and serviceability of the compounds such as the nature and graininess of the abrasive , the quantity of the compound added to the container at a time are investigated .
	manualset3
138688	7	407271	5	NULL	NULL	NULL	NULL	abrasive 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Some factors affecting the capacity and serviceability of the compounds such as the nature and graininess of the abrasive , the quantity of the compound added to the container at a time are investigated .
	manualset3
138689	8	407271	5	NULL	NULL	0	NULL	quantity 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some factors affecting the capacity and serviceability of the compounds such as the nature and graininess of the abrasive , the quantity of the compound added to the container at a time are investigated .
	manualset3
138690	9	407271	5	NULL	NULL	0	NULL	compound 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Some factors affecting the capacity and serviceability of the compounds such as the nature and graininess of the abrasive , the quantity of the compound added to the container at a time are investigated .
	manualset3
138691	10	407271	5	NULL	NULL	0	NULL	container 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Some factors affecting the capacity and serviceability of the compounds such as the nature and graininess of the abrasive , the quantity of the compound added to the container at a time are investigated .
	manualset3
138692	11	407271	5	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Some factors affecting the capacity and serviceability of the compounds such as the nature and graininess of the abrasive , the quantity of the compound added to the container at a time are investigated .
	manualset3
138693	1	407272	5	NULL	NULL	0	NULL	partial loss 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A partial loss of CD2 and CD5 in the predominant CD3 T-cell lymphocytes suggested a clonal proliferation .
	manualset3
138694	2	407272	5	NULL	NULL	0	NULL	CD2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A partial loss of CD2 and CD5 in the predominant CD3 T-cell lymphocytes suggested a clonal proliferation .
	manualset3
138695	3	407272	5	NULL	NULL	0	NULL	CD5 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A partial loss of CD2 and CD5 in the predominant CD3 T-cell lymphocytes suggested a clonal proliferation .
	manualset3
138696	4	407272	5	NULL	NULL	0	NULL	CD3 T-cell lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A partial loss of CD2 and CD5 in the predominant CD3 T-cell lymphocytes suggested a clonal proliferation .
	manualset3
138697	5	407272	5	NULL	NULL	0	NULL	clonal proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A partial loss of CD2 and CD5 in the predominant CD3 T-cell lymphocytes suggested a clonal proliferation .
	manualset3
138698	1	407273	5	NULL	NULL	0	NULL	factors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some factors affecting the cytotoxic immune reaction of rat mast cells .
	manualset3
138699	2	407273	5	NULL	NULL	0	NULL	cytotoxic immune reaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Some factors affecting the cytotoxic immune reaction of rat mast cells .
	manualset3
138700	3	407273	5	NULL	NULL	0	NULL	rat mast cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Some factors affecting the cytotoxic immune reaction of rat mast cells .
	manualset3
138701	1	407274	5	NULL	NULL	0	NULL	PrP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Some features of the PrP , however , are similar to structures found in aggregating proteins , such as the wheat glutenin , keratin , and collagen .
	manualset3
138702	2	407274	5	NULL	NULL	0	NULL	structures 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some features of the PrP , however , are similar to structures found in aggregating proteins , such as the wheat glutenin , keratin , and collagen .
	manualset3
138703	3	407274	5	NULL	NULL	0	NULL	aggregating proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Some features of the PrP , however , are similar to structures found in aggregating proteins , such as the wheat glutenin , keratin , and collagen .
	manualset3
138704	4	407274	5	NULL	NULL	0	NULL	wheat glutenin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Some features of the PrP , however , are similar to structures found in aggregating proteins , such as the wheat glutenin , keratin , and collagen .
	manualset3
138705	5	407274	5	NULL	NULL	0	NULL	keratin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Some features of the PrP , however , are similar to structures found in aggregating proteins , such as the wheat glutenin , keratin , and collagen .
	manualset3
138706	6	407274	5	NULL	NULL	0	NULL	collagen 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Some features of the PrP , however , are similar to structures found in aggregating proteins , such as the wheat glutenin , keratin , and collagen .
	manualset3
138707	1	407275	5	NULL	NULL	0	NULL	ligand binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Some ligand binding , including part of that in the upper stratum griseum superficiale , apparently survived such lesions .
	manualset3
138708	2	407275	5	NULL	NULL	0	NULL	upper stratum griseum superficiale	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Some ligand binding , including part of that in the upper stratum griseum superficiale , apparently survived such lesions .
	manualset3
138709	3	407275	5	NULL	NULL	0	NULL	lesions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Some ligand binding , including part of that in the upper stratum griseum superficiale , apparently survived such lesions .
	manualset3
138710	1	407276	5	NULL	NULL	0	NULL	methodological aspects	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some methodological aspects and characteristics on analysis of bone and liver alkaline phosphatase ( EC 3.1.3.1 , ALP ) isoforms by high-performance liquid chromatography ( HPLC ) methods are presented .
	manualset3
138711	2	407276	5	NULL	NULL	0	NULL	characteristics 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some methodological aspects and characteristics on analysis of bone and liver alkaline phosphatase ( EC 3.1.3.1 , ALP ) isoforms by high-performance liquid chromatography ( HPLC ) methods are presented .
	manualset3
138712	3	407276	5	NULL	NULL	0	NULL	analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some methodological aspects and characteristics on analysis of bone and liver alkaline phosphatase ( EC 3.1.3.1 , ALP ) isoforms by high-performance liquid chromatography ( HPLC ) methods are presented .
	manualset3
138713	4	407276	5	NULL	NULL	NULL	NULL	bone alkaline phosphatase ( EC 3.1.3.1 , ALP ) isoforms	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Some methodological aspects and characteristics on analysis of bone and liver alkaline phosphatase ( EC 3.1.3.1 , ALP ) isoforms by high-performance liquid chromatography ( HPLC ) methods are presented .
	manualset3
138714	5	407276	5	NULL	NULL	0	NULL	liver alkaline phosphatase ( EC 3.1.3.1 , ALP ) isoforms	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Some methodological aspects and characteristics on analysis of bone and liver alkaline phosphatase ( EC 3.1.3.1 , ALP ) isoforms by high-performance liquid chromatography ( HPLC ) methods are presented .
	manualset3
138715	6	407276	5	NULL	NULL	0	NULL	high-performance liquid chromatography ( HPLC ) methods 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some methodological aspects and characteristics on analysis of bone and liver alkaline phosphatase ( EC 3.1.3.1 , ALP ) isoforms by high-performance liquid chromatography ( HPLC ) methods are presented .
	manualset3
138716	1	407277	5	NULL	NULL	0	NULL	metric indices 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some metric indices for the assessment of land consolidation projects .
	manualset3
138717	2	407277	5	NULL	NULL	0	NULL	assessment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some metric indices for the assessment of land consolidation projects .
	manualset3
138718	3	407277	5	NULL	NULL	NULL	NULL	land consolidation projects 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Some metric indices for the assessment of land consolidation projects .
	manualset3
138719	1	407278	5	NULL	NULL	0	NULL	models 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Some models focus on development of receptive fields while others focus on the structure of cortical maps , i.e. , the arrangement of receptive field properties across the cortex .
	manualset3
138720	2	407278	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some models focus on development of receptive fields while others focus on the structure of cortical maps , i.e. , the arrangement of receptive field properties across the cortex .
	manualset3
138721	3	407278	5	NULL	NULL	0	NULL	receptive fields	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Some models focus on development of receptive fields while others focus on the structure of cortical maps , i.e. , the arrangement of receptive field properties across the cortex .
	manualset3
138722	4	407278	5	NULL	NULL	0	NULL	structure 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some models focus on development of receptive fields while others focus on the structure of cortical maps , i.e. , the arrangement of receptive field properties across the cortex .
	manualset3
138723	5	407278	5	NULL	NULL	0	NULL	cortical maps	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Some models focus on development of receptive fields while others focus on the structure of cortical maps , i.e. , the arrangement of receptive field properties across the cortex .
	manualset3
138724	6	407278	5	NULL	NULL	0	NULL	arrangement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some models focus on development of receptive fields while others focus on the structure of cortical maps , i.e. , the arrangement of receptive field properties across the cortex .
	manualset3
138725	7	407278	5	NULL	NULL	0	NULL	receptive field properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some models focus on development of receptive fields while others focus on the structure of cortical maps , i.e. , the arrangement of receptive field properties across the cortex .
	manualset3
138726	8	407278	5	NULL	NULL	0	NULL	cortex 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Some models focus on development of receptive fields while others focus on the structure of cortical maps , i.e. , the arrangement of receptive field properties across the cortex .
	manualset3
138727	1	407279	5	NULL	NULL	0	NULL	TgAA-positive sera	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Some of the TgAA-positive sera of patients reacted with 25 kDa peptide in addition to three tryptic peptides above .
	manualset3
138728	2	407279	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Some of the TgAA-positive sera of patients reacted with 25 kDa peptide in addition to three tryptic peptides above .
	manualset3
138729	3	407279	5	NULL	NULL	0	NULL	25 kDa peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Some of the TgAA-positive sera of patients reacted with 25 kDa peptide in addition to three tryptic peptides above .
	manualset3
138730	4	407279	5	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some of the TgAA-positive sera of patients reacted with 25 kDa peptide in addition to three tryptic peptides above .
	manualset3
138731	5	407279	5	NULL	NULL	0	NULL	three 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Some of the TgAA-positive sera of patients reacted with 25 kDa peptide in addition to three tryptic peptides above .
	manualset3
138732	6	407279	5	NULL	NULL	0	NULL	tryptic peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Some of the TgAA-positive sera of patients reacted with 25 kDa peptide in addition to three tryptic peptides above .
	manualset3
138733	1	407280	5	NULL	NULL	0	NULL	past history	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A past history of hysterical fits and neurotic depression was found in 3 cases ( 12.5 % ) and 2 cases ( 8.3 % ) respectively .
	manualset3
138734	2	407280	5	NULL	NULL	0	NULL	hysterical fits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A past history of hysterical fits and neurotic depression was found in 3 cases ( 12.5 % ) and 2 cases ( 8.3 % ) respectively .
	manualset3
138735	3	407280	5	NULL	NULL	0	NULL	neurotic depression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A past history of hysterical fits and neurotic depression was found in 3 cases ( 12.5 % ) and 2 cases ( 8.3 % ) respectively .
	manualset3
138736	4	407280	5	NULL	NULL	0	NULL	3 cases	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A past history of hysterical fits and neurotic depression was found in 3 cases ( 12.5 % ) and 2 cases ( 8.3 % ) respectively .
	manualset3
138737	5	407280	5	NULL	NULL	0	NULL	 12.5 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A past history of hysterical fits and neurotic depression was found in 3 cases ( 12.5 % ) and 2 cases ( 8.3 % ) respectively .
	manualset3
138738	6	407280	5	NULL	NULL	0	NULL	2 cases	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A past history of hysterical fits and neurotic depression was found in 3 cases ( 12.5 % ) and 2 cases ( 8.3 % ) respectively .
	manualset3
138739	7	407280	5	NULL	NULL	0	NULL	 8.3 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A past history of hysterical fits and neurotic depression was found in 3 cases ( 12.5 % ) and 2 cases ( 8.3 % ) respectively .
	manualset3
138740	1	407281	5	NULL	NULL	0	NULL	organizational system 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some of the organizational and professional system forces structuring their attitudes and actions were grant-related time lines , administrative burdens , and team turnover .
	manualset3
138741	2	407281	5	NULL	NULL	0	NULL	professional system 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some of the organizational and professional system forces structuring their attitudes and actions were grant-related time lines , administrative burdens , and team turnover .
	manualset3
138742	3	407281	5	NULL	NULL	0	NULL	attitudes 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Some of the organizational and professional system forces structuring their attitudes and actions were grant-related time lines , administrative burdens , and team turnover .
	manualset3
138743	4	407281	5	NULL	NULL	0	NULL	actions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some of the organizational and professional system forces structuring their attitudes and actions were grant-related time lines , administrative burdens , and team turnover .
	manualset3
138744	5	407281	5	NULL	NULL	0	NULL	grant-related time lines	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Some of the organizational and professional system forces structuring their attitudes and actions were grant-related time lines , administrative burdens , and team turnover .
	manualset3
138745	6	407281	5	NULL	NULL	0	NULL	administrative burdens	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some of the organizational and professional system forces structuring their attitudes and actions were grant-related time lines , administrative burdens , and team turnover .
	manualset3
138746	7	407281	5	NULL	NULL	0	NULL	team turnover	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some of the organizational and professional system forces structuring their attitudes and actions were grant-related time lines , administrative burdens , and team turnover .
	manualset3
138747	1	407282	5	NULL	NULL	0	NULL	cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Some of these cases showed a marked increase in levels of anti-STE-C during the course of the disease .
	manualset3
138748	2	407282	5	NULL	NULL	0	NULL	levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some of these cases showed a marked increase in levels of anti-STE-C during the course of the disease .
	manualset3
138749	3	407282	5	NULL	NULL	0	NULL	anti-STE-C	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Some of these cases showed a marked increase in levels of anti-STE-C during the course of the disease .
	manualset3
138750	4	407282	5	NULL	NULL	0	NULL	course 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some of these cases showed a marked increase in levels of anti-STE-C during the course of the disease .
	manualset3
138751	5	407282	5	NULL	NULL	0	NULL	disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Some of these cases showed a marked increase in levels of anti-STE-C during the course of the disease .
	manualset3
138752	1	407283	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Some patients seem to have a psychological sensitivity that predisposes them to react with pain catastrophizing after amputation of a limb , and this coping style may contribute to increased facilitation , impaired modulation of nociceptive signals , or both .
	manualset3
138753	2	407283	5	NULL	NULL	0	NULL	psychological sensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Some patients seem to have a psychological sensitivity that predisposes them to react with pain catastrophizing after amputation of a limb , and this coping style may contribute to increased facilitation , impaired modulation of nociceptive signals , or both .
	manualset3
138754	3	407283	5	NULL	NULL	0	NULL	pain 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Some patients seem to have a psychological sensitivity that predisposes them to react with pain catastrophizing after amputation of a limb , and this coping style may contribute to increased facilitation , impaired modulation of nociceptive signals , or both .
	manualset3
138755	4	407283	5	NULL	NULL	0	NULL	amputation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some patients seem to have a psychological sensitivity that predisposes them to react with pain catastrophizing after amputation of a limb , and this coping style may contribute to increased facilitation , impaired modulation of nociceptive signals , or both .
	manualset3
138756	5	407283	5	NULL	NULL	0	NULL	limb 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Some patients seem to have a psychological sensitivity that predisposes them to react with pain catastrophizing after amputation of a limb , and this coping style may contribute to increased facilitation , impaired modulation of nociceptive signals , or both .
	manualset3
138757	6	407283	5	NULL	NULL	0	NULL	coping style 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some patients seem to have a psychological sensitivity that predisposes them to react with pain catastrophizing after amputation of a limb , and this coping style may contribute to increased facilitation , impaired modulation of nociceptive signals , or both .
	manualset3
138758	7	407283	5	NULL	NULL	0	NULL	facilitation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some patients seem to have a psychological sensitivity that predisposes them to react with pain catastrophizing after amputation of a limb , and this coping style may contribute to increased facilitation , impaired modulation of nociceptive signals , or both .
	manualset3
138759	8	407283	5	NULL	NULL	0	NULL	impaired modulation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Some patients seem to have a psychological sensitivity that predisposes them to react with pain catastrophizing after amputation of a limb , and this coping style may contribute to increased facilitation , impaired modulation of nociceptive signals , or both .
	manualset3
138760	9	407283	5	NULL	NULL	0	NULL	nociceptive signals 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Some patients seem to have a psychological sensitivity that predisposes them to react with pain catastrophizing after amputation of a limb , and this coping style may contribute to increased facilitation , impaired modulation of nociceptive signals , or both .
	manualset3
138761	1	407284	5	NULL	NULL	0	NULL	starting points 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some possible starting points for a truly Canadian ethic for dentistry are suggested from a non-dentist , physician ethicist .
	manualset3
138762	2	407284	5	NULL	NULL	0	NULL	truly Canadian ethic	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some possible starting points for a truly Canadian ethic for dentistry are suggested from a non-dentist , physician ethicist .
	manualset3
138763	3	407284	5	NULL	NULL	0	NULL	dentistry 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some possible starting points for a truly Canadian ethic for dentistry are suggested from a non-dentist , physician ethicist .
	manualset3
138764	4	407284	5	NULL	NULL	0	NULL	non-dentist , physician ethicist	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Some possible starting points for a truly Canadian ethic for dentistry are suggested from a non-dentist , physician ethicist .
	manualset3
138765	1	407285	5	NULL	NULL	0	NULL	paste root canal treatment material	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A paste root canal treatment material used at the time of maxillary root canal treatment had leaked out of the root canal in both patients .
	manualset3
138766	2	407285	5	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	A paste root canal treatment material used at the time of maxillary root canal treatment had leaked out of the root canal in both patients .
	manualset3
138767	3	407285	5	NULL	NULL	0	NULL	maxillary root canal treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A paste root canal treatment material used at the time of maxillary root canal treatment had leaked out of the root canal in both patients .
	manualset3
138768	4	407285	5	NULL	NULL	0	NULL	root canal	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A paste root canal treatment material used at the time of maxillary root canal treatment had leaked out of the root canal in both patients .
	manualset3
138769	5	407285	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A paste root canal treatment material used at the time of maxillary root canal treatment had leaked out of the root canal in both patients .
	manualset3
138770	1	407286	5	NULL	NULL	0	NULL	pro-apoptotic bcl-family members 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Some pro-apoptotic bcl-family members , including Hrk , may contribute to the delayed hypersensitive reaction in AIDS , in macrophages eliminating opportunistic infection .
	manualset3
138771	2	407286	5	NULL	NULL	0	NULL	Hrk 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Some pro-apoptotic bcl-family members , including Hrk , may contribute to the delayed hypersensitive reaction in AIDS , in macrophages eliminating opportunistic infection .
	manualset3
138772	3	407286	5	NULL	NULL	0	NULL	delayed hypersensitive reaction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Some pro-apoptotic bcl-family members , including Hrk , may contribute to the delayed hypersensitive reaction in AIDS , in macrophages eliminating opportunistic infection .
	manualset3
138773	4	407286	5	NULL	NULL	0	NULL	AIDS 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Some pro-apoptotic bcl-family members , including Hrk , may contribute to the delayed hypersensitive reaction in AIDS , in macrophages eliminating opportunistic infection .
	manualset3
138774	5	407286	5	NULL	NULL	0	NULL	macrophages eliminating opportunistic infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Some pro-apoptotic bcl-family members , including Hrk , may contribute to the delayed hypersensitive reaction in AIDS , in macrophages eliminating opportunistic infection .
	manualset3
138775	1	407287	5	NULL	NULL	0	NULL	properties 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some properties of phagocytic cells .
	manualset3
138776	2	407287	5	NULL	NULL	0	NULL	phagocytic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Some properties of phagocytic cells .
	manualset3
138777	1	407288	5	NULL	NULL	0	NULL	reaction products 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some reaction products were also found in the rough endoplasmic reticulum and/or nuclear envelope , suggesting that ChE is synthesized by Schwann cells .
	manualset3
138778	2	407288	5	NULL	NULL	0	NULL	rough endoplasmic reticulum	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Some reaction products were also found in the rough endoplasmic reticulum and/or nuclear envelope , suggesting that ChE is synthesized by Schwann cells .
	manualset3
138779	3	407288	5	NULL	NULL	0	NULL	nuclear envelope	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Some reaction products were also found in the rough endoplasmic reticulum and/or nuclear envelope , suggesting that ChE is synthesized by Schwann cells .
	manualset3
138780	4	407288	5	NULL	NULL	0	NULL	ChE 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Some reaction products were also found in the rough endoplasmic reticulum and/or nuclear envelope , suggesting that ChE is synthesized by Schwann cells .
	manualset3
138781	5	407288	5	NULL	NULL	0	NULL	Schwann cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Some reaction products were also found in the rough endoplasmic reticulum and/or nuclear envelope , suggesting that ChE is synthesized by Schwann cells .
	manualset3
138782	1	407289	5	NULL	NULL	0	NULL	educational models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Some recent educational models ( Schon 's reflection-in-action and reflective practicums ( 1 ) , Boisot 's E-space ( 2 ) , Kolb 's learning cycle ( 3 ) ) provide for a more comprehensive and complete view of health professional education .
	manualset3
138783	2	407289	5	NULL	NULL	0	NULL	Schon 's reflection-in-action	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Some recent educational models ( Schon 's reflection-in-action and reflective practicums ( 1 ) , Boisot 's E-space ( 2 ) , Kolb 's learning cycle ( 3 ) ) provide for a more comprehensive and complete view of health professional education .
	manualset3
138784	3	407289	5	NULL	NULL	0	NULL	reflective practicums	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Some recent educational models ( Schon 's reflection-in-action and reflective practicums ( 1 ) , Boisot 's E-space ( 2 ) , Kolb 's learning cycle ( 3 ) ) provide for a more comprehensive and complete view of health professional education .
	manualset3
138785	4	407289	5	NULL	NULL	0	NULL	Boisot 's E-space	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Some recent educational models ( Schon 's reflection-in-action and reflective practicums ( 1 ) , Boisot 's E-space ( 2 ) , Kolb 's learning cycle ( 3 ) ) provide for a more comprehensive and complete view of health professional education .
	manualset3
138786	5	407289	5	NULL	NULL	0	NULL	Kolb 's learning cycle	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Some recent educational models ( Schon 's reflection-in-action and reflective practicums ( 1 ) , Boisot 's E-space ( 2 ) , Kolb 's learning cycle ( 3 ) ) provide for a more comprehensive and complete view of health professional education .
	manualset3
138787	6	407289	5	NULL	NULL	0	NULL	comprehensive and complete view	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some recent educational models ( Schon 's reflection-in-action and reflective practicums ( 1 ) , Boisot 's E-space ( 2 ) , Kolb 's learning cycle ( 3 ) ) provide for a more comprehensive and complete view of health professional education .
	manualset3
138788	7	407289	5	NULL	NULL	0	NULL	health professional education	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some recent educational models ( Schon 's reflection-in-action and reflective practicums ( 1 ) , Boisot 's E-space ( 2 ) , Kolb 's learning cycle ( 3 ) ) provide for a more comprehensive and complete view of health professional education .
	manualset3
138789	1	407290	5	NULL	NULL	0	NULL	recommendations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some recommendations are made in what respects the diagnosis and evaluation of patients with Streptococcus bovis infective endocarditis .
	manualset3
138790	2	407290	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Some recommendations are made in what respects the diagnosis and evaluation of patients with Streptococcus bovis infective endocarditis .
	manualset3
138791	3	407290	5	NULL	NULL	0	NULL	evaluation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Some recommendations are made in what respects the diagnosis and evaluation of patients with Streptococcus bovis infective endocarditis .
	manualset3
138792	4	407290	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Some recommendations are made in what respects the diagnosis and evaluation of patients with Streptococcus bovis infective endocarditis .
	manualset3
138793	5	407290	5	NULL	NULL	0	NULL	Streptococcus bovis infective endocarditis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Some recommendations are made in what respects the diagnosis and evaluation of patients with Streptococcus bovis infective endocarditis .
	manualset3
138794	1	407291	5	NULL	NULL	0	NULL	range 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some remarks on the range of validity of the model by hallstrom and davis .
	manualset3
138795	2	407291	5	NULL	NULL	0	NULL	validity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some remarks on the range of validity of the model by hallstrom and davis .
	manualset3
138796	3	407291	5	NULL	NULL	0	NULL	model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Some remarks on the range of validity of the model by hallstrom and davis .
	manualset3
138797	4	407291	5	NULL	NULL	0	NULL	hallstrom 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Some remarks on the range of validity of the model by hallstrom and davis .
	manualset3
138798	5	407291	5	NULL	NULL	0	NULL	davis 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Some remarks on the range of validity of the model by hallstrom and davis .
	manualset3
138799	1	407292	5	NULL	NULL	0	NULL	stratum granulosum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A patchy , discontinuous staining was also seen in stratum granulosum and corneum layers , which are not stained at all in control cultures .
	manualset3
138800	2	407292	5	NULL	NULL	0	NULL	corneum layers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A patchy , discontinuous staining was also seen in stratum granulosum and corneum layers , which are not stained at all in control cultures .
	manualset3
138801	3	407292	5	NULL	NULL	0	NULL	control cultures	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A patchy , discontinuous staining was also seen in stratum granulosum and corneum layers , which are not stained at all in control cultures .
	manualset3
138802	1	407293	5	NULL	NULL	0	NULL	restorative techniques	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Some restorative techniques for implant supported restorations will be familiar to dentists used to providing conventional crown and bridgework .
	manualset3
138803	2	407293	5	NULL	NULL	0	NULL	implant supported restorations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Some restorative techniques for implant supported restorations will be familiar to dentists used to providing conventional crown and bridgework .
	manualset3
138804	3	407293	5	NULL	NULL	0	NULL	dentists 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Some restorative techniques for implant supported restorations will be familiar to dentists used to providing conventional crown and bridgework .
	manualset3
138805	4	407293	5	NULL	NULL	NULL	NULL	conventional crown	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Some restorative techniques for implant supported restorations will be familiar to dentists used to providing conventional crown and bridgework .
	manualset3
142882	5	407293	5	NULL	NULL	0	NULL	bridgework 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Some restorative techniques for implant supported restorations will be familiar to dentists used to providing conventional crown and bridgework .
	manualset3
138806	1	407294	5	NULL	NULL	0	NULL	sesquiterpene lactones 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Some sesquiterpene lactones and related compounds were tested for anti-inflammatory activity in rodents .
	manualset3
138807	2	407294	5	NULL	NULL	0	NULL	related compounds	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Some sesquiterpene lactones and related compounds were tested for anti-inflammatory activity in rodents .
	manualset3
138808	3	407294	5	NULL	NULL	0	NULL	anti-inflammatory activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Some sesquiterpene lactones and related compounds were tested for anti-inflammatory activity in rodents .
	manualset3
138809	4	407294	5	NULL	NULL	0	NULL	rodents 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Some sesquiterpene lactones and related compounds were tested for anti-inflammatory activity in rodents .
	manualset3
138810	1	407295	5	NULL	NULL	0	NULL	species 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Some species inhabit the constant darkness of caves as well as the dim , natural photophase of rain-forests .
	manualset3
138811	2	407295	5	NULL	NULL	0	NULL	constant darkness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some species inhabit the constant darkness of caves as well as the dim , natural photophase of rain-forests .
	manualset3
138812	3	407295	5	NULL	NULL	0	NULL	caves 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Some species inhabit the constant darkness of caves as well as the dim , natural photophase of rain-forests .
	manualset3
138813	4	407295	5	NULL	NULL	0	NULL	natural photophase 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Some species inhabit the constant darkness of caves as well as the dim , natural photophase of rain-forests .
	manualset3
138814	5	407295	5	NULL	NULL	0	NULL	rain-forests	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Some species inhabit the constant darkness of caves as well as the dim , natural photophase of rain-forests .
	manualset3
138815	1	407296	5	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some studies have suggested that glutaminergic NMDA receptor activation in the inferior olive resulting in excitotoxic neuronal injury in the cerebellum is the underlying cause of posthypoxic myoclonus .
	manualset3
138816	2	407296	5	NULL	NULL	0	NULL	glutaminergic NMDA receptor activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Some studies have suggested that glutaminergic NMDA receptor activation in the inferior olive resulting in excitotoxic neuronal injury in the cerebellum is the underlying cause of posthypoxic myoclonus .
	manualset3
138817	3	407296	5	NULL	NULL	0	NULL	inferior olive 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Some studies have suggested that glutaminergic NMDA receptor activation in the inferior olive resulting in excitotoxic neuronal injury in the cerebellum is the underlying cause of posthypoxic myoclonus .
	manualset3
138818	4	407296	5	NULL	NULL	0	NULL	excitotoxic neuronal injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Some studies have suggested that glutaminergic NMDA receptor activation in the inferior olive resulting in excitotoxic neuronal injury in the cerebellum is the underlying cause of posthypoxic myoclonus .
	manualset3
138819	5	407296	5	NULL	NULL	0	NULL	cerebellum 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Some studies have suggested that glutaminergic NMDA receptor activation in the inferior olive resulting in excitotoxic neuronal injury in the cerebellum is the underlying cause of posthypoxic myoclonus .
	manualset3
138820	6	407296	5	NULL	NULL	0	NULL	posthypoxic myoclonus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Some studies have suggested that glutaminergic NMDA receptor activation in the inferior olive resulting in excitotoxic neuronal injury in the cerebellum is the underlying cause of posthypoxic myoclonus .
	manualset3
138821	1	407297	5	NULL	NULL	0	NULL	surgeons 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Some surgeons who employ the anterior approach facilitate exposure of the joint capsule by elevation of the origins of the sartorius and rectus femoris muscles .
	manualset3
138822	2	407297	5	NULL	NULL	0	NULL	anterior approach	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Some surgeons who employ the anterior approach facilitate exposure of the joint capsule by elevation of the origins of the sartorius and rectus femoris muscles .
	manualset3
138823	3	407297	5	NULL	NULL	0	NULL	exposure 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Some surgeons who employ the anterior approach facilitate exposure of the joint capsule by elevation of the origins of the sartorius and rectus femoris muscles .
	manualset3
138824	4	407297	5	NULL	NULL	0	NULL	joint capsule 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Some surgeons who employ the anterior approach facilitate exposure of the joint capsule by elevation of the origins of the sartorius and rectus femoris muscles .
	manualset3
138825	5	407297	5	NULL	NULL	0	NULL	elevation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some surgeons who employ the anterior approach facilitate exposure of the joint capsule by elevation of the origins of the sartorius and rectus femoris muscles .
	manualset3
138826	6	407297	5	NULL	NULL	0	NULL	origins 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some surgeons who employ the anterior approach facilitate exposure of the joint capsule by elevation of the origins of the sartorius and rectus femoris muscles .
	manualset3
138827	7	407297	5	NULL	NULL	0	NULL	sartorius muscles 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Some surgeons who employ the anterior approach facilitate exposure of the joint capsule by elevation of the origins of the sartorius and rectus femoris muscles .
	manualset3
138828	8	407297	5	NULL	NULL	0	NULL	rectus femoris muscles 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Some surgeons who employ the anterior approach facilitate exposure of the joint capsule by elevation of the origins of the sartorius and rectus femoris muscles .
	manualset3
138829	1	407298	5	NULL	NULL	0	NULL	useful aspects 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some useful aspects of such a system are discussed , particularly those which make for easier biologist-user interaction and system extensibility .
	manualset3
138830	2	407298	5	NULL	NULL	0	NULL	system 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some useful aspects of such a system are discussed , particularly those which make for easier biologist-user interaction and system extensibility .
	manualset3
138831	3	407298	5	NULL	NULL	0	NULL	biologist-user interaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some useful aspects of such a system are discussed , particularly those which make for easier biologist-user interaction and system extensibility .
	manualset3
138832	4	407298	5	NULL	NULL	0	NULL	system extensibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some useful aspects of such a system are discussed , particularly those which make for easier biologist-user interaction and system extensibility .
	manualset3
138833	1	407299	5	NULL	NULL	0	NULL	heavily stained cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Some very heavily stained cells showed a distribution and morphology similar to ED-2-positive macrophages which were abundant during early stages of EAN .
	manualset3
138834	2	407299	5	NULL	NULL	0	NULL	distribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some very heavily stained cells showed a distribution and morphology similar to ED-2-positive macrophages which were abundant during early stages of EAN .
	manualset3
138835	3	407299	5	NULL	NULL	0	NULL	morphology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some very heavily stained cells showed a distribution and morphology similar to ED-2-positive macrophages which were abundant during early stages of EAN .
	manualset3
138836	4	407299	5	NULL	NULL	0	NULL	ED-2-positive macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Some very heavily stained cells showed a distribution and morphology similar to ED-2-positive macrophages which were abundant during early stages of EAN .
	manualset3
138837	5	407299	5	NULL	NULL	0	NULL	early stages 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Some very heavily stained cells showed a distribution and morphology similar to ED-2-positive macrophages which were abundant during early stages of EAN .
	manualset3
138838	6	407299	5	NULL	NULL	0	NULL	EAN 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some very heavily stained cells showed a distribution and morphology similar to ED-2-positive macrophages which were abundant during early stages of EAN .
	manualset3
138839	1	407300	5	NULL	NULL	0	NULL	Cerebral hemorrhage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cerebral hemorrhage from unsuspected intracranial tumors ) .
	manualset3
138840	2	407300	5	NULL	NULL	0	NULL	unsuspected intracranial tumors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cerebral hemorrhage from unsuspected intracranial tumors ) .
	manualset3
138841	1	407301	5	NULL	NULL	0	NULL	pathoadaptive deletion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A pathoadaptive deletion in an enteroaggregative Escherichia coli outbreak strain enhances virulence in a Caenorhabditis elegans model .
	manualset3
138842	2	407301	5	NULL	NULL	0	NULL	enteroaggregative Escherichia coli outbreak strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A pathoadaptive deletion in an enteroaggregative Escherichia coli outbreak strain enhances virulence in a Caenorhabditis elegans model .
	manualset3
138843	3	407301	5	NULL	NULL	0	NULL	virulence 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A pathoadaptive deletion in an enteroaggregative Escherichia coli outbreak strain enhances virulence in a Caenorhabditis elegans model .
	manualset3
138844	4	407301	5	NULL	NULL	0	NULL	Caenorhabditis elegans model	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A pathoadaptive deletion in an enteroaggregative Escherichia coli outbreak strain enhances virulence in a Caenorhabditis elegans model .
	manualset3
138845	1	407302	5	NULL	NULL	NULL	NULL	quality 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Somewhat unexpectedly , the quality of the social environment of the nursing home was found to be as important as attitudes toward job benefits in accounting for institutional loyalty .
	manualset3
138846	2	407302	5	NULL	NULL	0	NULL	social environment	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Somewhat unexpectedly , the quality of the social environment of the nursing home was found to be as important as attitudes toward job benefits in accounting for institutional loyalty .
	manualset3
138847	3	407302	5	NULL	NULL	0	NULL	nursing home	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Somewhat unexpectedly , the quality of the social environment of the nursing home was found to be as important as attitudes toward job benefits in accounting for institutional loyalty .
	manualset3
138848	4	407302	5	NULL	NULL	0	NULL	attitudes 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Somewhat unexpectedly , the quality of the social environment of the nursing home was found to be as important as attitudes toward job benefits in accounting for institutional loyalty .
	manualset3
138849	5	407302	5	NULL	NULL	0	NULL	job benefits	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Somewhat unexpectedly , the quality of the social environment of the nursing home was found to be as important as attitudes toward job benefits in accounting for institutional loyalty .
	manualset3
138850	6	407302	5	NULL	NULL	0	NULL	institutional loyalty	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Somewhat unexpectedly , the quality of the social environment of the nursing home was found to be as important as attitudes toward job benefits in accounting for institutional loyalty .
	manualset3
138851	1	407303	5	NULL	NULL	0	NULL	Sonography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Sonography during early pregnancy : dependence of threshold and discriminatory values on transvaginal transducer frequency .
	manualset3
138852	2	407303	5	NULL	NULL	0	NULL	early pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sonography during early pregnancy : dependence of threshold and discriminatory values on transvaginal transducer frequency .
	manualset3
138853	3	407303	5	NULL	NULL	0	NULL	dependence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sonography during early pregnancy : dependence of threshold and discriminatory values on transvaginal transducer frequency .
	manualset3
138854	4	407303	5	NULL	NULL	0	NULL	threshold 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sonography during early pregnancy : dependence of threshold and discriminatory values on transvaginal transducer frequency .
	manualset3
138855	5	407303	5	NULL	NULL	0	NULL	discriminatory values 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sonography during early pregnancy : dependence of threshold and discriminatory values on transvaginal transducer frequency .
	manualset3
138856	6	407303	5	NULL	NULL	0	NULL	transvaginal transducer frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sonography during early pregnancy : dependence of threshold and discriminatory values on transvaginal transducer frequency .
	manualset3
138857	1	407304	5	NULL	NULL	0	NULL	admission 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Soon after admission he developed ventricular fibrillation with no other cause than this severe hypercalcemia .
	manualset3
138858	2	407304	5	NULL	NULL	0	NULL	ventricular fibrillation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Soon after admission he developed ventricular fibrillation with no other cause than this severe hypercalcemia .
	manualset3
138859	3	407304	5	NULL	NULL	0	NULL	severe hypercalcemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Soon after admission he developed ventricular fibrillation with no other cause than this severe hypercalcemia .
	manualset3
138860	1	407305	5	NULL	NULL	0	NULL	Sorption 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sorption is one of the fundamental processes controlling the transport and availability of nitroaromatics , but previous studies have focused mainly on sorption to model clay minerals , whereas little attention has been paid to the sorptive interactions with natural soils .
	manualset3
138861	2	407305	5	NULL	NULL	0	NULL	fundamental processes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sorption is one of the fundamental processes controlling the transport and availability of nitroaromatics , but previous studies have focused mainly on sorption to model clay minerals , whereas little attention has been paid to the sorptive interactions with natural soils .
	manualset3
138862	3	407305	5	NULL	NULL	0	NULL	availability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sorption is one of the fundamental processes controlling the transport and availability of nitroaromatics , but previous studies have focused mainly on sorption to model clay minerals , whereas little attention has been paid to the sorptive interactions with natural soils .
	manualset3
138863	4	407305	5	NULL	NULL	0	NULL	nitroaromatics 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sorption is one of the fundamental processes controlling the transport and availability of nitroaromatics , but previous studies have focused mainly on sorption to model clay minerals , whereas little attention has been paid to the sorptive interactions with natural soils .
	manualset3
138864	5	407305	5	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sorption is one of the fundamental processes controlling the transport and availability of nitroaromatics , but previous studies have focused mainly on sorption to model clay minerals , whereas little attention has been paid to the sorptive interactions with natural soils .
	manualset3
138865	6	407305	5	NULL	NULL	0	NULL	sorption 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sorption is one of the fundamental processes controlling the transport and availability of nitroaromatics , but previous studies have focused mainly on sorption to model clay minerals , whereas little attention has been paid to the sorptive interactions with natural soils .
	manualset3
138866	7	407305	5	NULL	NULL	0	NULL	clay minerals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sorption is one of the fundamental processes controlling the transport and availability of nitroaromatics , but previous studies have focused mainly on sorption to model clay minerals , whereas little attention has been paid to the sorptive interactions with natural soils .
	manualset3
138867	8	407305	5	NULL	NULL	0	NULL	attention 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sorption is one of the fundamental processes controlling the transport and availability of nitroaromatics , but previous studies have focused mainly on sorption to model clay minerals , whereas little attention has been paid to the sorptive interactions with natural soils .
	manualset3
138868	9	407305	5	NULL	NULL	0	NULL	sorptive interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sorption is one of the fundamental processes controlling the transport and availability of nitroaromatics , but previous studies have focused mainly on sorption to model clay minerals , whereas little attention has been paid to the sorptive interactions with natural soils .
	manualset3
138869	10	407305	5	NULL	NULL	0	NULL	natural soils	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Sorption is one of the fundamental processes controlling the transport and availability of nitroaromatics , but previous studies have focused mainly on sorption to model clay minerals , whereas little attention has been paid to the sorptive interactions with natural soils .
	manualset3
142883	11	407305	5	NULL	NULL	0	NULL	transport 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sorption is one of the fundamental processes controlling the transport and availability of nitroaromatics , but previous studies have focused mainly on sorption to model clay minerals , whereas little attention has been paid to the sorptive interactions with natural soils .
	manualset3
138870	1	407306	5	NULL	NULL	0	NULL	Sostdc1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sostdc1 , a secreted inhibitor of the Wnt and Bmp pathways , also regulates the spatial patterning of teeth and hair .
	manualset3
138871	2	407306	5	NULL	NULL	0	NULL	secreted inhibitor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sostdc1 , a secreted inhibitor of the Wnt and Bmp pathways , also regulates the spatial patterning of teeth and hair .
	manualset3
138872	3	407306	5	NULL	NULL	0	NULL	Wnt pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sostdc1 , a secreted inhibitor of the Wnt and Bmp pathways , also regulates the spatial patterning of teeth and hair .
	manualset3
138873	4	407306	5	NULL	NULL	0	NULL	Bmp pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sostdc1 , a secreted inhibitor of the Wnt and Bmp pathways , also regulates the spatial patterning of teeth and hair .
	manualset3
138874	5	407306	5	NULL	NULL	NULL	NULL	spatial patterning	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Sostdc1 , a secreted inhibitor of the Wnt and Bmp pathways , also regulates the spatial patterning of teeth and hair .
	manualset3
138875	6	407306	5	NULL	NULL	0	NULL	teeth 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Sostdc1 , a secreted inhibitor of the Wnt and Bmp pathways , also regulates the spatial patterning of teeth and hair .
	manualset3
138876	7	407306	5	NULL	NULL	0	NULL	hair 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Sostdc1 , a secreted inhibitor of the Wnt and Bmp pathways , also regulates the spatial patterning of teeth and hair .
	manualset3
138877	1	407307	5	NULL	NULL	0	NULL	Sound speed	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sound speed in water-saturated glass beads as a function of frequency and porosity .
	manualset3
138878	2	407307	5	NULL	NULL	0	NULL	water-saturated glass beads 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sound speed in water-saturated glass beads as a function of frequency and porosity .
	manualset3
138879	3	407307	5	NULL	NULL	0	NULL	function 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sound speed in water-saturated glass beads as a function of frequency and porosity .
	manualset3
138880	4	407307	5	NULL	NULL	0	NULL	frequency 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sound speed in water-saturated glass beads as a function of frequency and porosity .
	manualset3
138881	5	407307	5	NULL	NULL	0	NULL	porosity 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sound speed in water-saturated glass beads as a function of frequency and porosity .
	manualset3
138882	1	407308	5	NULL	NULL	0	NULL	Southern and colony hybridization analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Southern and colony hybridization analyses indicated that the invH gene is present in all Salmonella strains tested ( 91 strains belonging to 37 serotypes ) with the exception of strains of Salmonella arizonae .
	manualset3
138883	2	407308	5	NULL	NULL	0	NULL	invH gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Southern and colony hybridization analyses indicated that the invH gene is present in all Salmonella strains tested ( 91 strains belonging to 37 serotypes ) with the exception of strains of Salmonella arizonae .
	manualset3
138884	3	407308	5	NULL	NULL	0	NULL	Salmonella strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Southern and colony hybridization analyses indicated that the invH gene is present in all Salmonella strains tested ( 91 strains belonging to 37 serotypes ) with the exception of strains of Salmonella arizonae .
	manualset3
138885	4	407308	5	NULL	NULL	0	NULL	 91 strains	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Southern and colony hybridization analyses indicated that the invH gene is present in all Salmonella strains tested ( 91 strains belonging to 37 serotypes ) with the exception of strains of Salmonella arizonae .
	manualset3
138886	5	407308	5	NULL	NULL	0	NULL	37 serotypes	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Southern and colony hybridization analyses indicated that the invH gene is present in all Salmonella strains tested ( 91 strains belonging to 37 serotypes ) with the exception of strains of Salmonella arizonae .
	manualset3
138887	6	407308	5	NULL	NULL	0	NULL	exception 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Southern and colony hybridization analyses indicated that the invH gene is present in all Salmonella strains tested ( 91 strains belonging to 37 serotypes ) with the exception of strains of Salmonella arizonae .
	manualset3
138888	7	407308	5	NULL	NULL	0	NULL	strains of Salmonella arizonae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Southern and colony hybridization analyses indicated that the invH gene is present in all Salmonella strains tested ( 91 strains belonging to 37 serotypes ) with the exception of strains of Salmonella arizonae .
	manualset3
138889	1	407309	5	NULL	NULL	0	NULL	Soviet science aide	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Soviet science aide ousted by United States .
	manualset3
138890	2	407309	5	NULL	NULL	0	NULL	United States	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Soviet science aide ousted by United States .
	manualset3
138891	1	407310	5	NULL	NULL	0	NULL	Soy 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Soy , vitamin E , and herbal remedies were the most common alternative therapies reported by participants ; use was greater in cases compared to controls .
	manualset3
138892	2	407310	5	NULL	NULL	0	NULL	vitamin E	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Soy , vitamin E , and herbal remedies were the most common alternative therapies reported by participants ; use was greater in cases compared to controls .
	manualset3
138893	3	407310	5	NULL	NULL	0	NULL	herbal remedies 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Soy , vitamin E , and herbal remedies were the most common alternative therapies reported by participants ; use was greater in cases compared to controls .
	manualset3
138894	4	407310	5	NULL	NULL	0	NULL	alternative therapies 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Soy , vitamin E , and herbal remedies were the most common alternative therapies reported by participants ; use was greater in cases compared to controls .
	manualset3
138895	5	407310	5	NULL	NULL	0	NULL	participants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Soy , vitamin E , and herbal remedies were the most common alternative therapies reported by participants ; use was greater in cases compared to controls .
	manualset3
138896	6	407310	5	NULL	NULL	0	NULL	cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Soy , vitamin E , and herbal remedies were the most common alternative therapies reported by participants ; use was greater in cases compared to controls .
	manualset3
138897	7	407310	5	NULL	NULL	0	NULL	controls 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Soy , vitamin E , and herbal remedies were the most common alternative therapies reported by participants ; use was greater in cases compared to controls .
	manualset3
138898	1	407311	5	NULL	NULL	0	NULL	Soya protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Soya protein attenuates abnormalities of the renin-angiotensin system in adipose tissue from obese rats .
	manualset3
138899	2	407311	5	NULL	NULL	0	NULL	abnormalities 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Soya protein attenuates abnormalities of the renin-angiotensin system in adipose tissue from obese rats .
	manualset3
138900	3	407311	5	NULL	NULL	0	NULL	renin-angiotensin system	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Soya protein attenuates abnormalities of the renin-angiotensin system in adipose tissue from obese rats .
	manualset3
138901	4	407311	5	NULL	NULL	0	NULL	adipose tissue 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Soya protein attenuates abnormalities of the renin-angiotensin system in adipose tissue from obese rats .
	manualset3
138902	5	407311	5	NULL	NULL	0	NULL	obese rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Soya protein attenuates abnormalities of the renin-angiotensin system in adipose tissue from obese rats .
	manualset3
138903	1	407312	5	NULL	NULL	0	NULL	Soybean plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Soybean plants can form tripartite symbiotic associations with rhizobia and arbuscular mycorrhizal ( AM ) fungi , but little is known about effects of co-inoculation with rhizobia and AM fungi on plant growth , or their relationships to root architecture as well as nitrogen ( N ) and phosphorus ( P ) availability .
	manualset3
138904	2	407312	5	NULL	NULL	NULL	NULL	tripartite symbiotic associations	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Soybean plants can form tripartite symbiotic associations with rhizobia and arbuscular mycorrhizal ( AM ) fungi , but little is known about effects of co-inoculation with rhizobia and AM fungi on plant growth , or their relationships to root architecture as well as nitrogen ( N ) and phosphorus ( P ) availability .
	manualset3
138905	3	407312	5	NULL	NULL	0	NULL	rhizobia 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Soybean plants can form tripartite symbiotic associations with rhizobia and arbuscular mycorrhizal ( AM ) fungi , but little is known about effects of co-inoculation with rhizobia and AM fungi on plant growth , or their relationships to root architecture as well as nitrogen ( N ) and phosphorus ( P ) availability .
	manualset3
138906	4	407312	5	NULL	NULL	0	NULL	arbuscular mycorrhizal ( AM ) fungi	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Soybean plants can form tripartite symbiotic associations with rhizobia and arbuscular mycorrhizal ( AM ) fungi , but little is known about effects of co-inoculation with rhizobia and AM fungi on plant growth , or their relationships to root architecture as well as nitrogen ( N ) and phosphorus ( P ) availability .
	manualset3
138907	5	407312	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Soybean plants can form tripartite symbiotic associations with rhizobia and arbuscular mycorrhizal ( AM ) fungi , but little is known about effects of co-inoculation with rhizobia and AM fungi on plant growth , or their relationships to root architecture as well as nitrogen ( N ) and phosphorus ( P ) availability .
	manualset3
138908	6	407312	5	NULL	NULL	0	NULL	co-inoculation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Soybean plants can form tripartite symbiotic associations with rhizobia and arbuscular mycorrhizal ( AM ) fungi , but little is known about effects of co-inoculation with rhizobia and AM fungi on plant growth , or their relationships to root architecture as well as nitrogen ( N ) and phosphorus ( P ) availability .
	manualset3
138909	7	407312	5	NULL	NULL	0	NULL	AM fungi	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Soybean plants can form tripartite symbiotic associations with rhizobia and arbuscular mycorrhizal ( AM ) fungi , but little is known about effects of co-inoculation with rhizobia and AM fungi on plant growth , or their relationships to root architecture as well as nitrogen ( N ) and phosphorus ( P ) availability .
	manualset3
138910	8	407312	5	NULL	NULL	0	NULL	plant growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Soybean plants can form tripartite symbiotic associations with rhizobia and arbuscular mycorrhizal ( AM ) fungi , but little is known about effects of co-inoculation with rhizobia and AM fungi on plant growth , or their relationships to root architecture as well as nitrogen ( N ) and phosphorus ( P ) availability .
	manualset3
138911	9	407312	5	NULL	NULL	0	NULL	relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Soybean plants can form tripartite symbiotic associations with rhizobia and arbuscular mycorrhizal ( AM ) fungi , but little is known about effects of co-inoculation with rhizobia and AM fungi on plant growth , or their relationships to root architecture as well as nitrogen ( N ) and phosphorus ( P ) availability .
	manualset3
138912	10	407312	5	NULL	NULL	0	NULL	root architecture 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Soybean plants can form tripartite symbiotic associations with rhizobia and arbuscular mycorrhizal ( AM ) fungi , but little is known about effects of co-inoculation with rhizobia and AM fungi on plant growth , or their relationships to root architecture as well as nitrogen ( N ) and phosphorus ( P ) availability .
	manualset3
138913	11	407312	5	NULL	NULL	0	NULL	nitrogen ( N ) availability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Soybean plants can form tripartite symbiotic associations with rhizobia and arbuscular mycorrhizal ( AM ) fungi , but little is known about effects of co-inoculation with rhizobia and AM fungi on plant growth , or their relationships to root architecture as well as nitrogen ( N ) and phosphorus ( P ) availability .
	manualset3
138914	12	407312	5	NULL	NULL	0	NULL	phosphorus ( P ) availability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Soybean plants can form tripartite symbiotic associations with rhizobia and arbuscular mycorrhizal ( AM ) fungi , but little is known about effects of co-inoculation with rhizobia and AM fungi on plant growth , or their relationships to root architecture as well as nitrogen ( N ) and phosphorus ( P ) availability .
	manualset3
142884	13	407312	5	NULL	NULL	0	NULL	rhizobia 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Soybean plants can form tripartite symbiotic associations with rhizobia and arbuscular mycorrhizal ( AM ) fungi , but little is known about effects of co-inoculation with rhizobia and AM fungi on plant growth , or their relationships to root architecture as well as nitrogen ( N ) and phosphorus ( P ) availability .
	manualset3
138915	1	407313	5	NULL	NULL	0	NULL	Sp1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sp1king out cancer ( ... and fibrosis ? ) .
	manualset3
138916	2	407313	5	NULL	NULL	0	NULL	cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Sp1king out cancer ( ... and fibrosis ? ) .
	manualset3
138917	3	407313	5	NULL	NULL	0	NULL	fibrosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Sp1king out cancer ( ... and fibrosis ? ) .
	manualset3
138918	1	407314	5	NULL	NULL	0	NULL	Space-time decoupling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Space-time decoupling in the branching process in the mutant toile of the filamentous brown alga Ectocarpus siliculosus .
	manualset3
138919	2	407314	5	NULL	NULL	0	NULL	branching process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Space-time decoupling in the branching process in the mutant toile of the filamentous brown alga Ectocarpus siliculosus .
	manualset3
138920	3	407314	5	NULL	NULL	0	NULL	mutant toile	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Space-time decoupling in the branching process in the mutant toile of the filamentous brown alga Ectocarpus siliculosus .
	manualset3
138921	4	407314	5	NULL	NULL	0	NULL	filamentous brown alga Ectocarpus siliculosus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Space-time decoupling in the branching process in the mutant toile of the filamentous brown alga Ectocarpus siliculosus .
	manualset3
138922	1	407315	5	NULL	NULL	0	NULL	Space 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Space , time , and host evolution facilitate coexistence of competing bacteriophages : theory and experiment .
	manualset3
138923	2	407315	5	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Space , time , and host evolution facilitate coexistence of competing bacteriophages : theory and experiment .
	manualset3
138924	3	407315	5	NULL	NULL	0	NULL	host evolution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Space , time , and host evolution facilitate coexistence of competing bacteriophages : theory and experiment .
	manualset3
138925	4	407315	5	NULL	NULL	0	NULL	coexistence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Space , time , and host evolution facilitate coexistence of competing bacteriophages : theory and experiment .
	manualset3
138926	5	407315	5	NULL	NULL	0	NULL	competing bacteriophages	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Space , time , and host evolution facilitate coexistence of competing bacteriophages : theory and experiment .
	manualset3
138927	6	407315	5	NULL	NULL	0	NULL	theory 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Space , time , and host evolution facilitate coexistence of competing bacteriophages : theory and experiment .
	manualset3
138928	7	407315	5	NULL	NULL	0	NULL	experiment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Space , time , and host evolution facilitate coexistence of competing bacteriophages : theory and experiment .
	manualset3
138929	1	407316	5	NULL	NULL	0	NULL	Spacing 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Spacing , orientation , and curvature of PEL are assessed from sections through 47 other hooves and compared with the stress and displacement data .
	manualset3
138930	2	407316	5	NULL	NULL	0	NULL	orientation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Spacing , orientation , and curvature of PEL are assessed from sections through 47 other hooves and compared with the stress and displacement data .
	manualset3
138931	3	407316	5	NULL	NULL	0	NULL	curvature 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spacing , orientation , and curvature of PEL are assessed from sections through 47 other hooves and compared with the stress and displacement data .
	manualset3
138932	4	407316	5	NULL	NULL	0	NULL	PEL 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spacing , orientation , and curvature of PEL are assessed from sections through 47 other hooves and compared with the stress and displacement data .
	manualset3
138933	5	407316	5	NULL	NULL	0	NULL	sections 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spacing , orientation , and curvature of PEL are assessed from sections through 47 other hooves and compared with the stress and displacement data .
	manualset3
138934	6	407316	5	NULL	NULL	0	NULL	47 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Spacing , orientation , and curvature of PEL are assessed from sections through 47 other hooves and compared with the stress and displacement data .
	manualset3
138935	7	407316	5	NULL	NULL	0	NULL	hooves 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Spacing , orientation , and curvature of PEL are assessed from sections through 47 other hooves and compared with the stress and displacement data .
	manualset3
138936	8	407316	5	NULL	NULL	0	NULL	stress 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Spacing , orientation , and curvature of PEL are assessed from sections through 47 other hooves and compared with the stress and displacement data .
	manualset3
138937	9	407316	5	NULL	NULL	0	NULL	displacement data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Spacing , orientation , and curvature of PEL are assessed from sections through 47 other hooves and compared with the stress and displacement data .
	manualset3
138938	1	407317	5	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A patient with Proteus syndrome presented with lower gastrointestinal bleeding due to multiple colonic hemangiomas , a finding which has not been described previously in this syndrome .
	manualset3
138939	2	407317	5	NULL	NULL	0	NULL	Proteus syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A patient with Proteus syndrome presented with lower gastrointestinal bleeding due to multiple colonic hemangiomas , a finding which has not been described previously in this syndrome .
	manualset3
138940	3	407317	5	NULL	NULL	0	NULL	lower gastrointestinal bleeding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A patient with Proteus syndrome presented with lower gastrointestinal bleeding due to multiple colonic hemangiomas , a finding which has not been described previously in this syndrome .
	manualset3
138941	4	407317	5	NULL	NULL	0	NULL	multiple colonic hemangiomas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A patient with Proteus syndrome presented with lower gastrointestinal bleeding due to multiple colonic hemangiomas , a finding which has not been described previously in this syndrome .
	manualset3
138942	5	407317	5	NULL	NULL	0	NULL	finding 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A patient with Proteus syndrome presented with lower gastrointestinal bleeding due to multiple colonic hemangiomas , a finding which has not been described previously in this syndrome .
	manualset3
138943	6	407317	5	NULL	NULL	0	NULL	syndrome 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A patient with Proteus syndrome presented with lower gastrointestinal bleeding due to multiple colonic hemangiomas , a finding which has not been described previously in this syndrome .
	manualset3
138944	1	407318	5	NULL	NULL	0	NULL	representation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sparse representation via 1-minimization for underdetermined systems in classification of tumors with gene expression data .
	manualset3
138945	2	407318	5	NULL	NULL	0	NULL	1-minimization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sparse representation via 1-minimization for underdetermined systems in classification of tumors with gene expression data .
	manualset3
138946	3	407318	5	NULL	NULL	0	NULL	underdetermined systems	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sparse representation via 1-minimization for underdetermined systems in classification of tumors with gene expression data .
	manualset3
138947	4	407318	5	NULL	NULL	0	NULL	classification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sparse representation via 1-minimization for underdetermined systems in classification of tumors with gene expression data .
	manualset3
138948	5	407318	5	NULL	NULL	0	NULL	tumors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sparse representation via 1-minimization for underdetermined systems in classification of tumors with gene expression data .
	manualset3
138949	6	407318	5	NULL	NULL	0	NULL	gene expression data	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Sparse representation via 1-minimization for underdetermined systems in classification of tumors with gene expression data .
	manualset3
138950	1	407319	5	NULL	NULL	0	NULL	Spasm 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Spasm of the near reflex , characterized by intermittent convergence , accommodation , and miosis , is a functional disturbance .
	manualset3
138951	2	407319	5	NULL	NULL	0	NULL	reflex 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Spasm of the near reflex , characterized by intermittent convergence , accommodation , and miosis , is a functional disturbance .
	manualset3
138952	3	407319	5	NULL	NULL	0	NULL	intermittent convergence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Spasm of the near reflex , characterized by intermittent convergence , accommodation , and miosis , is a functional disturbance .
	manualset3
138953	4	407319	5	NULL	NULL	0	NULL	accommodation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Spasm of the near reflex , characterized by intermittent convergence , accommodation , and miosis , is a functional disturbance .
	manualset3
138954	5	407319	5	NULL	NULL	NULL	NULL	miosis 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Spasm of the near reflex , characterized by intermittent convergence , accommodation , and miosis , is a functional disturbance .
	manualset3
138955	6	407319	5	NULL	NULL	0	NULL	functional disturbance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Spasm of the near reflex , characterized by intermittent convergence , accommodation , and miosis , is a functional disturbance .
	manualset3
138956	1	407320	5	NULL	NULL	0	NULL	Spatial correlates 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatial , behavioral and sensory correlates of hippocampal CA1 complex spike cell activity : implications for information processing functions .
	manualset3
138957	2	407320	5	NULL	NULL	0	NULL	behavioral correlates 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatial , behavioral and sensory correlates of hippocampal CA1 complex spike cell activity : implications for information processing functions .
	manualset3
138958	3	407320	5	NULL	NULL	0	NULL	sensory correlates 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatial , behavioral and sensory correlates of hippocampal CA1 complex spike cell activity : implications for information processing functions .
	manualset3
138959	4	407320	5	NULL	NULL	0	NULL	hippocampal CA1 complex spike cell activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatial , behavioral and sensory correlates of hippocampal CA1 complex spike cell activity : implications for information processing functions .
	manualset3
138960	5	407320	5	NULL	NULL	0	NULL	implications 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatial , behavioral and sensory correlates of hippocampal CA1 complex spike cell activity : implications for information processing functions .
	manualset3
138961	6	407320	5	NULL	NULL	0	NULL	information processing functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatial , behavioral and sensory correlates of hippocampal CA1 complex spike cell activity : implications for information processing functions .
	manualset3
138962	1	407321	5	NULL	NULL	0	NULL	Spatial Fourier transformation	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatial Fourier transformation is applied to the fluorescence intensity recorded at various times after bleaching of a narrow rectangular area within an image representative of the film .
	manualset3
138963	2	407321	5	NULL	NULL	0	NULL	fluorescence intensity 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatial Fourier transformation is applied to the fluorescence intensity recorded at various times after bleaching of a narrow rectangular area within an image representative of the film .
	manualset3
138964	3	407321	5	NULL	NULL	0	NULL	times 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatial Fourier transformation is applied to the fluorescence intensity recorded at various times after bleaching of a narrow rectangular area within an image representative of the film .
	manualset3
138965	4	407321	5	NULL	NULL	0	NULL	narrow rectangular area	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatial Fourier transformation is applied to the fluorescence intensity recorded at various times after bleaching of a narrow rectangular area within an image representative of the film .
	manualset3
138966	5	407321	5	NULL	NULL	0	NULL	image representative	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatial Fourier transformation is applied to the fluorescence intensity recorded at various times after bleaching of a narrow rectangular area within an image representative of the film .
	manualset3
138967	6	407321	5	NULL	NULL	0	NULL	film 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatial Fourier transformation is applied to the fluorescence intensity recorded at various times after bleaching of a narrow rectangular area within an image representative of the film .
	manualset3
138968	1	407322	5	NULL	NULL	0	NULL	Spatial localization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatial localization of the coenzyme FAD in the protein structure : hot-tritium bombardment and ESR experiments .
	manualset3
138969	2	407322	5	NULL	NULL	0	NULL	coenzyme FAD	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatial localization of the coenzyme FAD in the protein structure : hot-tritium bombardment and ESR experiments .
	manualset3
138970	3	407322	5	NULL	NULL	0	NULL	protein structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatial localization of the coenzyme FAD in the protein structure : hot-tritium bombardment and ESR experiments .
	manualset3
138971	4	407322	5	NULL	NULL	0	NULL	hot-tritium bombardment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatial localization of the coenzyme FAD in the protein structure : hot-tritium bombardment and ESR experiments .
	manualset3
138972	5	407322	5	NULL	NULL	0	NULL	ESR experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatial localization of the coenzyme FAD in the protein structure : hot-tritium bombardment and ESR experiments .
	manualset3
138973	1	407323	5	NULL	NULL	0	NULL	Spatial scaling 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatial scaling of microbial eukaryote diversity .
	manualset3
138974	2	407323	5	NULL	NULL	0	NULL	microbial eukaryote diversity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatial scaling of microbial eukaryote diversity .
	manualset3
138975	1	407324	5	NULL	NULL	0	NULL	Spatial speckle intensity correlations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatial speckle intensity correlations are used to determine the spatial Fourier magnitude of a field incident on a random scattering medium .
	manualset3
138976	2	407324	5	NULL	NULL	0	NULL	spatial Fourier magnitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatial speckle intensity correlations are used to determine the spatial Fourier magnitude of a field incident on a random scattering medium .
	manualset3
138977	3	407324	5	NULL	NULL	0	NULL	field incident	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatial speckle intensity correlations are used to determine the spatial Fourier magnitude of a field incident on a random scattering medium .
	manualset3
138978	4	407324	5	NULL	NULL	0	NULL	random scattering medium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatial speckle intensity correlations are used to determine the spatial Fourier magnitude of a field incident on a random scattering medium .
	manualset3
138979	1	407325	5	NULL	NULL	0	NULL	Spatially resolved ( 19 ) F nuclear magnetic resonance ( NMR ) spin-lattice relaxation rates 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatially resolved ( 19 ) F and ( 7 ) Li nuclear magnetic resonance ( NMR ) spin-lattice relaxation rates have been measured in LiF crystals irradiated with 1.44 GeV Xe ions at fluences from 10 ( 10 ) to 10 ( 12 ) ionscm ( -2 ) .
	manualset3
138980	2	407325	5	NULL	NULL	0	NULL	Spatially resolved ( 7 ) Li nuclear magnetic resonance ( NMR ) spin-lattice relaxation rates 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatially resolved ( 19 ) F and ( 7 ) Li nuclear magnetic resonance ( NMR ) spin-lattice relaxation rates have been measured in LiF crystals irradiated with 1.44 GeV Xe ions at fluences from 10 ( 10 ) to 10 ( 12 ) ionscm ( -2 ) .
	manualset3
138981	3	407325	5	NULL	NULL	0	NULL	LiF crystals 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatially resolved ( 19 ) F and ( 7 ) Li nuclear magnetic resonance ( NMR ) spin-lattice relaxation rates have been measured in LiF crystals irradiated with 1.44 GeV Xe ions at fluences from 10 ( 10 ) to 10 ( 12 ) ionscm ( -2 ) .
	manualset3
138982	4	407325	5	NULL	NULL	0	NULL	1.44 GeV Xe ions 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatially resolved ( 19 ) F and ( 7 ) Li nuclear magnetic resonance ( NMR ) spin-lattice relaxation rates have been measured in LiF crystals irradiated with 1.44 GeV Xe ions at fluences from 10 ( 10 ) to 10 ( 12 ) ionscm ( -2 ) .
	manualset3
138983	5	407325	5	NULL	NULL	0	NULL	fluences 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatially resolved ( 19 ) F and ( 7 ) Li nuclear magnetic resonance ( NMR ) spin-lattice relaxation rates have been measured in LiF crystals irradiated with 1.44 GeV Xe ions at fluences from 10 ( 10 ) to 10 ( 12 ) ionscm ( -2 ) .
	manualset3
138984	6	407325	5	NULL	NULL	0	NULL	 10 ( 10 ) to 10 ( 12 ) ionscm ( -2 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatially resolved ( 19 ) F and ( 7 ) Li nuclear magnetic resonance ( NMR ) spin-lattice relaxation rates have been measured in LiF crystals irradiated with 1.44 GeV Xe ions at fluences from 10 ( 10 ) to 10 ( 12 ) ionscm ( -2 ) .
	manualset3
138985	1	407326	5	NULL	NULL	0	NULL	attention 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention centered over the possible contribution of cytokines to the destabilization of the plaque .
	manualset3
138986	2	407326	5	NULL	NULL	0	NULL	possible contribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention centered over the possible contribution of cytokines to the destabilization of the plaque .
	manualset3
138987	3	407326	5	NULL	NULL	0	NULL	cytokines 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention centered over the possible contribution of cytokines to the destabilization of the plaque .
	manualset3
138988	4	407326	5	NULL	NULL	0	NULL	destabilization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention centered over the possible contribution of cytokines to the destabilization of the plaque .
	manualset3
138989	5	407326	5	NULL	NULL	0	NULL	plaque 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention centered over the possible contribution of cytokines to the destabilization of the plaque .
	manualset3
138990	1	407327	5	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A patient with acute nonlymphocytic leukemia developed a painful scrotal ulcer thought initially to be caused by infection .
	manualset3
138991	2	407327	5	NULL	NULL	0	NULL	acute nonlymphocytic leukemia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A patient with acute nonlymphocytic leukemia developed a painful scrotal ulcer thought initially to be caused by infection .
	manualset3
138992	3	407327	5	NULL	NULL	0	NULL	painful scrotal ulcer	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A patient with acute nonlymphocytic leukemia developed a painful scrotal ulcer thought initially to be caused by infection .
	manualset3
138993	4	407327	5	NULL	NULL	0	NULL	thought 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A patient with acute nonlymphocytic leukemia developed a painful scrotal ulcer thought initially to be caused by infection .
	manualset3
138994	5	407327	5	NULL	NULL	0	NULL	infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A patient with acute nonlymphocytic leukemia developed a painful scrotal ulcer thought initially to be caused by infection .
	manualset3
138995	1	407328	5	NULL	NULL	0	NULL	Special attention 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention is focused on one age-graded association with an examination of recruitment , participation , and attrition over a 6-year period .
	manualset3
138996	2	407328	5	NULL	NULL	0	NULL	one 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention is focused on one age-graded association with an examination of recruitment , participation , and attrition over a 6-year period .
	manualset3
138997	3	407328	5	NULL	NULL	0	NULL	age-graded association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention is focused on one age-graded association with an examination of recruitment , participation , and attrition over a 6-year period .
	manualset3
138998	4	407328	5	NULL	NULL	0	NULL	examination 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention is focused on one age-graded association with an examination of recruitment , participation , and attrition over a 6-year period .
	manualset3
138999	5	407328	5	NULL	NULL	0	NULL	recruitment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention is focused on one age-graded association with an examination of recruitment , participation , and attrition over a 6-year period .
	manualset3
139000	6	407328	5	NULL	NULL	0	NULL	participation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention is focused on one age-graded association with an examination of recruitment , participation , and attrition over a 6-year period .
	manualset3
139001	7	407328	5	NULL	NULL	0	NULL	attrition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention is focused on one age-graded association with an examination of recruitment , participation , and attrition over a 6-year period .
	manualset3
139002	8	407328	5	NULL	NULL	0	NULL	6-year period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention is focused on one age-graded association with an examination of recruitment , participation , and attrition over a 6-year period .
	manualset3
139003	9	407328	5	NULL	NULL	0	NULL	6-year period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention is focused on one age-graded association with an examination of recruitment , participation , and attrition over a 6-year period .
	manualset3
139004	1	407329	5	NULL	NULL	0	NULL	Special attention 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention is given to newly emerging Asian historical demography where different source materials require different methods and techniques , which in turn are expected to broaden the scope of the so far disproportionality fertility-oriented field .
	manualset3
139005	2	407329	5	NULL	NULL	0	NULL	Asian historical demography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention is given to newly emerging Asian historical demography where different source materials require different methods and techniques , which in turn are expected to broaden the scope of the so far disproportionality fertility-oriented field .
	manualset3
139006	3	407329	5	NULL	NULL	0	NULL	source materials 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention is given to newly emerging Asian historical demography where different source materials require different methods and techniques , which in turn are expected to broaden the scope of the so far disproportionality fertility-oriented field .
	manualset3
139007	4	407329	5	NULL	NULL	0	NULL	different methods	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention is given to newly emerging Asian historical demography where different source materials require different methods and techniques , which in turn are expected to broaden the scope of the so far disproportionality fertility-oriented field .
	manualset3
139008	5	407329	5	NULL	NULL	0	NULL	techniques 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention is given to newly emerging Asian historical demography where different source materials require different methods and techniques , which in turn are expected to broaden the scope of the so far disproportionality fertility-oriented field .
	manualset3
139009	6	407329	5	NULL	NULL	0	NULL	scope 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention is given to newly emerging Asian historical demography where different source materials require different methods and techniques , which in turn are expected to broaden the scope of the so far disproportionality fertility-oriented field .
	manualset3
139010	1	407330	5	NULL	NULL	0	NULL	Special attention	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention is given to the present status of diagnostic methods , the author pointing out the nonspecificity of individual signs and symptoms of the disease .
	manualset3
139011	2	407330	5	NULL	NULL	0	NULL	status 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention is given to the present status of diagnostic methods , the author pointing out the nonspecificity of individual signs and symptoms of the disease .
	manualset3
139012	3	407330	5	NULL	NULL	0	NULL	diagnostic methods	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention is given to the present status of diagnostic methods , the author pointing out the nonspecificity of individual signs and symptoms of the disease .
	manualset3
139013	4	407330	5	NULL	NULL	0	NULL	author 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention is given to the present status of diagnostic methods , the author pointing out the nonspecificity of individual signs and symptoms of the disease .
	manualset3
139014	5	407330	5	NULL	NULL	0	NULL	nonspecificity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention is given to the present status of diagnostic methods , the author pointing out the nonspecificity of individual signs and symptoms of the disease .
	manualset3
139015	6	407330	5	NULL	NULL	0	NULL	individual signs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention is given to the present status of diagnostic methods , the author pointing out the nonspecificity of individual signs and symptoms of the disease .
	manualset3
139016	7	407330	5	NULL	NULL	0	NULL	symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention is given to the present status of diagnostic methods , the author pointing out the nonspecificity of individual signs and symptoms of the disease .
	manualset3
139017	8	407330	5	NULL	NULL	0	NULL	disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention is given to the present status of diagnostic methods , the author pointing out the nonspecificity of individual signs and symptoms of the disease .
	manualset3
139018	1	407331	5	NULL	NULL	0	NULL	Special attention	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention must be focused on the concentrations of ALA heptyl ester ; as excess may lead to cytotoxicity and inefficient PpIX generation .
	manualset3
139019	2	407331	5	NULL	NULL	0	NULL	concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention must be focused on the concentrations of ALA heptyl ester ; as excess may lead to cytotoxicity and inefficient PpIX generation .
	manualset3
139020	3	407331	5	NULL	NULL	0	NULL	 ALA heptyl ester	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention must be focused on the concentrations of ALA heptyl ester ; as excess may lead to cytotoxicity and inefficient PpIX generation .
	manualset3
139021	4	407331	5	NULL	NULL	0	NULL	cytotoxicity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention must be focused on the concentrations of ALA heptyl ester ; as excess may lead to cytotoxicity and inefficient PpIX generation .
	manualset3
139022	5	407331	5	NULL	NULL	0	NULL	inefficient PpIX generation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention must be focused on the concentrations of ALA heptyl ester ; as excess may lead to cytotoxicity and inefficient PpIX generation .
	manualset3
139023	1	407332	5	NULL	NULL	0	NULL	emphasis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Special emphasis is laid on the variety of organic manifestations and on the fact that bioptic investigations have not resulted in typical findings leading to diagnosis .
	manualset3
139024	2	407332	5	NULL	NULL	0	NULL	variety 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Special emphasis is laid on the variety of organic manifestations and on the fact that bioptic investigations have not resulted in typical findings leading to diagnosis .
	manualset3
139025	3	407332	5	NULL	NULL	0	NULL	organic manifestations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Special emphasis is laid on the variety of organic manifestations and on the fact that bioptic investigations have not resulted in typical findings leading to diagnosis .
	manualset3
139026	4	407332	5	NULL	NULL	0	NULL	bioptic investigations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Special emphasis is laid on the variety of organic manifestations and on the fact that bioptic investigations have not resulted in typical findings leading to diagnosis .
	manualset3
139027	5	407332	5	NULL	NULL	0	NULL	typical findings 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Special emphasis is laid on the variety of organic manifestations and on the fact that bioptic investigations have not resulted in typical findings leading to diagnosis .
	manualset3
139028	6	407332	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Special emphasis is laid on the variety of organic manifestations and on the fact that bioptic investigations have not resulted in typical findings leading to diagnosis .
	manualset3
139029	1	407333	5	NULL	NULL	0	NULL	emphasis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Special emphasis is placed on intravenous cannabinoid self-administration in squirrel monkeys , a valid , reliable and flexible model that we have developed over the past decade .
	manualset3
139030	2	407333	5	NULL	NULL	0	NULL	intravenous cannabinoid self-administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Special emphasis is placed on intravenous cannabinoid self-administration in squirrel monkeys , a valid , reliable and flexible model that we have developed over the past decade .
	manualset3
139031	3	407333	5	NULL	NULL	0	NULL	squirrel monkeys	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Special emphasis is placed on intravenous cannabinoid self-administration in squirrel monkeys , a valid , reliable and flexible model that we have developed over the past decade .
	manualset3
139032	4	407333	5	NULL	NULL	0	NULL	valid , reliable and flexible model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Special emphasis is placed on intravenous cannabinoid self-administration in squirrel monkeys , a valid , reliable and flexible model that we have developed over the past decade .
	manualset3
139033	5	407333	5	NULL	NULL	0	NULL	decade 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Special emphasis is placed on intravenous cannabinoid self-administration in squirrel monkeys , a valid , reliable and flexible model that we have developed over the past decade .
	manualset3
139034	1	407334	5	NULL	NULL	0	NULL	spectral responses	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specially , according to the spectral responses of HB , the microenvironments in biomolecules and liposomes could be set in a sequence of hydrophobic grades , i.e. , liposomes ) proteins ) polysaccharides .
	manualset3
139035	2	407334	5	NULL	NULL	0	NULL	HB 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Specially , according to the spectral responses of HB , the microenvironments in biomolecules and liposomes could be set in a sequence of hydrophobic grades , i.e. , liposomes ) proteins ) polysaccharides .
	manualset3
139036	3	407334	5	NULL	NULL	0	NULL	microenvironments 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Specially , according to the spectral responses of HB , the microenvironments in biomolecules and liposomes could be set in a sequence of hydrophobic grades , i.e. , liposomes ) proteins ) polysaccharides .
	manualset3
139037	4	407334	5	NULL	NULL	0	NULL	biomolecules 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Specially , according to the spectral responses of HB , the microenvironments in biomolecules and liposomes could be set in a sequence of hydrophobic grades , i.e. , liposomes ) proteins ) polysaccharides .
	manualset3
139038	5	407334	5	NULL	NULL	0	NULL	liposomes 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Specially , according to the spectral responses of HB , the microenvironments in biomolecules and liposomes could be set in a sequence of hydrophobic grades , i.e. , liposomes ) proteins ) polysaccharides .
	manualset3
139039	6	407334	5	NULL	NULL	0	NULL	sequence 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Specially , according to the spectral responses of HB , the microenvironments in biomolecules and liposomes could be set in a sequence of hydrophobic grades , i.e. , liposomes ) proteins ) polysaccharides .
	manualset3
139040	7	407334	5	NULL	NULL	0	NULL	hydrophobic grades 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Specially , according to the spectral responses of HB , the microenvironments in biomolecules and liposomes could be set in a sequence of hydrophobic grades , i.e. , liposomes ) proteins ) polysaccharides .
	manualset3
139041	8	407334	5	NULL	NULL	0	NULL	liposomes 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Specially , according to the spectral responses of HB , the microenvironments in biomolecules and liposomes could be set in a sequence of hydrophobic grades , i.e. , liposomes ) proteins ) polysaccharides .
	manualset3
139042	9	407334	5	NULL	NULL	0	NULL	proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Specially , according to the spectral responses of HB , the microenvironments in biomolecules and liposomes could be set in a sequence of hydrophobic grades , i.e. , liposomes ) proteins ) polysaccharides .
	manualset3
139043	10	407334	5	NULL	NULL	0	NULL	polysaccharides 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Specially , according to the spectral responses of HB , the microenvironments in biomolecules and liposomes could be set in a sequence of hydrophobic grades , i.e. , liposomes ) proteins ) polysaccharides .
	manualset3
139044	1	407335	5	NULL	NULL	0	NULL	neuronal bistability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Specially , neuronal bistability is equipped by after-depolarisation current .
	manualset3
139045	2	407335	5	NULL	NULL	NULL	NULL	after-depolarisation current 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Specially , neuronal bistability is equipped by after-depolarisation current .
	manualset3
139046	1	407336	5	NULL	NULL	0	NULL	Speciation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Speciation by polyploidization in these frogs has been the source of considerable debate , but the various published hypotheses have assumed that polyploids arose through either autopolyploidy or allopolyploidy of extant diploid species .
	manualset3
139047	2	407336	5	NULL	NULL	0	NULL	polyploidization 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Speciation by polyploidization in these frogs has been the source of considerable debate , but the various published hypotheses have assumed that polyploids arose through either autopolyploidy or allopolyploidy of extant diploid species .
	manualset3
139048	3	407336	5	NULL	NULL	0	NULL	frogs 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Speciation by polyploidization in these frogs has been the source of considerable debate , but the various published hypotheses have assumed that polyploids arose through either autopolyploidy or allopolyploidy of extant diploid species .
	manualset3
139049	4	407336	5	NULL	NULL	0	NULL	source 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Speciation by polyploidization in these frogs has been the source of considerable debate , but the various published hypotheses have assumed that polyploids arose through either autopolyploidy or allopolyploidy of extant diploid species .
	manualset3
139050	5	407336	5	NULL	NULL	0	NULL	published hypotheses	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Speciation by polyploidization in these frogs has been the source of considerable debate , but the various published hypotheses have assumed that polyploids arose through either autopolyploidy or allopolyploidy of extant diploid species .
	manualset3
139051	6	407336	5	NULL	NULL	0	NULL	polyploids 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Speciation by polyploidization in these frogs has been the source of considerable debate , but the various published hypotheses have assumed that polyploids arose through either autopolyploidy or allopolyploidy of extant diploid species .
	manualset3
139052	7	407336	5	NULL	NULL	0	NULL	autopolyploidy 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Speciation by polyploidization in these frogs has been the source of considerable debate , but the various published hypotheses have assumed that polyploids arose through either autopolyploidy or allopolyploidy of extant diploid species .
	manualset3
139053	8	407336	5	NULL	NULL	0	NULL	allopolyploidy 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Speciation by polyploidization in these frogs has been the source of considerable debate , but the various published hypotheses have assumed that polyploids arose through either autopolyploidy or allopolyploidy of extant diploid species .
	manualset3
139054	9	407336	5	NULL	NULL	0	NULL	diploid species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Speciation by polyploidization in these frogs has been the source of considerable debate , but the various published hypotheses have assumed that polyploids arose through either autopolyploidy or allopolyploidy of extant diploid species .
	manualset3
139055	1	407337	5	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A patient with subarachnoid hemorrhage was found to have electrocardiographic abnormalities resembling an acute myocardial infarction as well as left ventriculographic findings of cardiac dysfunction .
	manualset3
139056	2	407337	5	NULL	NULL	0	NULL	subarachnoid hemorrhage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A patient with subarachnoid hemorrhage was found to have electrocardiographic abnormalities resembling an acute myocardial infarction as well as left ventriculographic findings of cardiac dysfunction .
	manualset3
139057	3	407337	5	NULL	NULL	0	NULL	electrocardiographic abnormalities 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A patient with subarachnoid hemorrhage was found to have electrocardiographic abnormalities resembling an acute myocardial infarction as well as left ventriculographic findings of cardiac dysfunction .
	manualset3
139058	4	407337	5	NULL	NULL	0	NULL	acute myocardial infarction	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A patient with subarachnoid hemorrhage was found to have electrocardiographic abnormalities resembling an acute myocardial infarction as well as left ventriculographic findings of cardiac dysfunction .
	manualset3
139059	5	407337	5	NULL	NULL	0	NULL	left ventriculographic findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A patient with subarachnoid hemorrhage was found to have electrocardiographic abnormalities resembling an acute myocardial infarction as well as left ventriculographic findings of cardiac dysfunction .
	manualset3
139060	6	407337	5	NULL	NULL	0	NULL	cardiac dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A patient with subarachnoid hemorrhage was found to have electrocardiographic abnormalities resembling an acute myocardial infarction as well as left ventriculographic findings of cardiac dysfunction .
	manualset3
139061	1	407338	5	NULL	NULL	0	NULL	Species-level identification 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Species-level identification of clinical staphylococcal isolates based on polymerase chain reaction -- restriction fragment length polymorphism analysis of a partial groEL gene sequence .
	manualset3
139062	2	407338	5	NULL	NULL	0	NULL	staphylococcal isolates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Species-level identification of clinical staphylococcal isolates based on polymerase chain reaction -- restriction fragment length polymorphism analysis of a partial groEL gene sequence .
	manualset3
139063	3	407338	5	NULL	NULL	0	NULL	polymerase chain reaction -- restriction fragment length polymorphism analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Species-level identification of clinical staphylococcal isolates based on polymerase chain reaction -- restriction fragment length polymorphism analysis of a partial groEL gene sequence .
	manualset3
139064	4	407338	5	NULL	NULL	0	NULL	partial groEL gene sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Species-level identification of clinical staphylococcal isolates based on polymerase chain reaction -- restriction fragment length polymorphism analysis of a partial groEL gene sequence .
	manualset3
139065	1	407339	5	NULL	NULL	0	NULL	Species 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Species of Poaceae ( n = 3 ) , Bromeliaceae ( 5 ) , Apiaceae ( 6 ) , Araceae ( 2 ) , Urticaceae ( 1 ) , Marantaceae ( 1 ) , Arecaceae ( 1 ) , Dipsacaceae ( 1 ) and Cyperaceae ( 1 ) were identified as phytotelmata .
	manualset3
139066	2	407339	5	NULL	NULL	0	NULL	Poaceae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Species of Poaceae ( n = 3 ) , Bromeliaceae ( 5 ) , Apiaceae ( 6 ) , Araceae ( 2 ) , Urticaceae ( 1 ) , Marantaceae ( 1 ) , Arecaceae ( 1 ) , Dipsacaceae ( 1 ) and Cyperaceae ( 1 ) were identified as phytotelmata .
	manualset3
139067	3	407339	5	NULL	NULL	0	NULL	n = 3 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Species of Poaceae ( n = 3 ) , Bromeliaceae ( 5 ) , Apiaceae ( 6 ) , Araceae ( 2 ) , Urticaceae ( 1 ) , Marantaceae ( 1 ) , Arecaceae ( 1 ) , Dipsacaceae ( 1 ) and Cyperaceae ( 1 ) were identified as phytotelmata .
	manualset3
139068	4	407339	5	NULL	NULL	0	NULL	Bromeliaceae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Species of Poaceae ( n = 3 ) , Bromeliaceae ( 5 ) , Apiaceae ( 6 ) , Araceae ( 2 ) , Urticaceae ( 1 ) , Marantaceae ( 1 ) , Arecaceae ( 1 ) , Dipsacaceae ( 1 ) and Cyperaceae ( 1 ) were identified as phytotelmata .
	manualset3
139069	5	407339	5	NULL	NULL	0	NULL	5 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Species of Poaceae ( n = 3 ) , Bromeliaceae ( 5 ) , Apiaceae ( 6 ) , Araceae ( 2 ) , Urticaceae ( 1 ) , Marantaceae ( 1 ) , Arecaceae ( 1 ) , Dipsacaceae ( 1 ) and Cyperaceae ( 1 ) were identified as phytotelmata .
	manualset3
139070	6	407339	5	NULL	NULL	0	NULL	Apiaceae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Species of Poaceae ( n = 3 ) , Bromeliaceae ( 5 ) , Apiaceae ( 6 ) , Araceae ( 2 ) , Urticaceae ( 1 ) , Marantaceae ( 1 ) , Arecaceae ( 1 ) , Dipsacaceae ( 1 ) and Cyperaceae ( 1 ) were identified as phytotelmata .
	manualset3
139071	7	407339	5	NULL	NULL	0	NULL	6 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Species of Poaceae ( n = 3 ) , Bromeliaceae ( 5 ) , Apiaceae ( 6 ) , Araceae ( 2 ) , Urticaceae ( 1 ) , Marantaceae ( 1 ) , Arecaceae ( 1 ) , Dipsacaceae ( 1 ) and Cyperaceae ( 1 ) were identified as phytotelmata .
	manualset3
139072	8	407339	5	NULL	NULL	0	NULL	Araceae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Species of Poaceae ( n = 3 ) , Bromeliaceae ( 5 ) , Apiaceae ( 6 ) , Araceae ( 2 ) , Urticaceae ( 1 ) , Marantaceae ( 1 ) , Arecaceae ( 1 ) , Dipsacaceae ( 1 ) and Cyperaceae ( 1 ) were identified as phytotelmata .
	manualset3
139073	9	407339	5	NULL	NULL	0	NULL	2 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Species of Poaceae ( n = 3 ) , Bromeliaceae ( 5 ) , Apiaceae ( 6 ) , Araceae ( 2 ) , Urticaceae ( 1 ) , Marantaceae ( 1 ) , Arecaceae ( 1 ) , Dipsacaceae ( 1 ) and Cyperaceae ( 1 ) were identified as phytotelmata .
	manualset3
139074	10	407339	5	NULL	NULL	0	NULL	Urticaceae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Species of Poaceae ( n = 3 ) , Bromeliaceae ( 5 ) , Apiaceae ( 6 ) , Araceae ( 2 ) , Urticaceae ( 1 ) , Marantaceae ( 1 ) , Arecaceae ( 1 ) , Dipsacaceae ( 1 ) and Cyperaceae ( 1 ) were identified as phytotelmata .
	manualset3
139075	11	407339	5	NULL	NULL	0	NULL	1 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Species of Poaceae ( n = 3 ) , Bromeliaceae ( 5 ) , Apiaceae ( 6 ) , Araceae ( 2 ) , Urticaceae ( 1 ) , Marantaceae ( 1 ) , Arecaceae ( 1 ) , Dipsacaceae ( 1 ) and Cyperaceae ( 1 ) were identified as phytotelmata .
	manualset3
139076	12	407339	5	NULL	NULL	0	NULL	Marantaceae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Species of Poaceae ( n = 3 ) , Bromeliaceae ( 5 ) , Apiaceae ( 6 ) , Araceae ( 2 ) , Urticaceae ( 1 ) , Marantaceae ( 1 ) , Arecaceae ( 1 ) , Dipsacaceae ( 1 ) and Cyperaceae ( 1 ) were identified as phytotelmata .
	manualset3
139077	13	407339	5	NULL	NULL	0	NULL	1 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Species of Poaceae ( n = 3 ) , Bromeliaceae ( 5 ) , Apiaceae ( 6 ) , Araceae ( 2 ) , Urticaceae ( 1 ) , Marantaceae ( 1 ) , Arecaceae ( 1 ) , Dipsacaceae ( 1 ) and Cyperaceae ( 1 ) were identified as phytotelmata .
	manualset3
139078	14	407339	5	NULL	NULL	0	NULL	Arecaceae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Species of Poaceae ( n = 3 ) , Bromeliaceae ( 5 ) , Apiaceae ( 6 ) , Araceae ( 2 ) , Urticaceae ( 1 ) , Marantaceae ( 1 ) , Arecaceae ( 1 ) , Dipsacaceae ( 1 ) and Cyperaceae ( 1 ) were identified as phytotelmata .
	manualset3
139079	15	407339	5	NULL	NULL	0	NULL	1 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Species of Poaceae ( n = 3 ) , Bromeliaceae ( 5 ) , Apiaceae ( 6 ) , Araceae ( 2 ) , Urticaceae ( 1 ) , Marantaceae ( 1 ) , Arecaceae ( 1 ) , Dipsacaceae ( 1 ) and Cyperaceae ( 1 ) were identified as phytotelmata .
	manualset3
139080	16	407339	5	NULL	NULL	0	NULL	Dipsacaceae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Species of Poaceae ( n = 3 ) , Bromeliaceae ( 5 ) , Apiaceae ( 6 ) , Araceae ( 2 ) , Urticaceae ( 1 ) , Marantaceae ( 1 ) , Arecaceae ( 1 ) , Dipsacaceae ( 1 ) and Cyperaceae ( 1 ) were identified as phytotelmata .
	manualset3
139081	17	407339	5	NULL	NULL	0	NULL	1 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Species of Poaceae ( n = 3 ) , Bromeliaceae ( 5 ) , Apiaceae ( 6 ) , Araceae ( 2 ) , Urticaceae ( 1 ) , Marantaceae ( 1 ) , Arecaceae ( 1 ) , Dipsacaceae ( 1 ) and Cyperaceae ( 1 ) were identified as phytotelmata .
	manualset3
139082	18	407339	5	NULL	NULL	0	NULL	Cyperaceae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Species of Poaceae ( n = 3 ) , Bromeliaceae ( 5 ) , Apiaceae ( 6 ) , Araceae ( 2 ) , Urticaceae ( 1 ) , Marantaceae ( 1 ) , Arecaceae ( 1 ) , Dipsacaceae ( 1 ) and Cyperaceae ( 1 ) were identified as phytotelmata .
	manualset3
139083	19	407339	5	NULL	NULL	0	NULL	1 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Species of Poaceae ( n = 3 ) , Bromeliaceae ( 5 ) , Apiaceae ( 6 ) , Araceae ( 2 ) , Urticaceae ( 1 ) , Marantaceae ( 1 ) , Arecaceae ( 1 ) , Dipsacaceae ( 1 ) and Cyperaceae ( 1 ) were identified as phytotelmata .
	manualset3
139084	20	407339	5	NULL	NULL	0	NULL	phytotelmata 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Species of Poaceae ( n = 3 ) , Bromeliaceae ( 5 ) , Apiaceae ( 6 ) , Araceae ( 2 ) , Urticaceae ( 1 ) , Marantaceae ( 1 ) , Arecaceae ( 1 ) , Dipsacaceae ( 1 ) and Cyperaceae ( 1 ) were identified as phytotelmata .
	manualset3
139085	1	407340	5	NULL	NULL	0	NULL	CD8 + T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific CD8 + T cells are induced during infection and evidence exist that they contribute to the elimination of parasites , an effect probably resulting from the Interferon gamma that they release .
	manualset3
139086	2	407340	5	NULL	NULL	0	NULL	infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific CD8 + T cells are induced during infection and evidence exist that they contribute to the elimination of parasites , an effect probably resulting from the Interferon gamma that they release .
	manualset3
139087	3	407340	5	NULL	NULL	0	NULL	evidence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific CD8 + T cells are induced during infection and evidence exist that they contribute to the elimination of parasites , an effect probably resulting from the Interferon gamma that they release .
	manualset3
139088	4	407340	5	NULL	NULL	0	NULL	elimination 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific CD8 + T cells are induced during infection and evidence exist that they contribute to the elimination of parasites , an effect probably resulting from the Interferon gamma that they release .
	manualset3
139089	5	407340	5	NULL	NULL	0	NULL	parasites 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific CD8 + T cells are induced during infection and evidence exist that they contribute to the elimination of parasites , an effect probably resulting from the Interferon gamma that they release .
	manualset3
139090	6	407340	5	NULL	NULL	0	NULL	Interferon gamma	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific CD8 + T cells are induced during infection and evidence exist that they contribute to the elimination of parasites , an effect probably resulting from the Interferon gamma that they release .
	manualset3
139693	7	407340	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific CD8 + T cells are induced during infection and evidence exist that they contribute to the elimination of parasites , an effect probably resulting from the Interferon gamma that they release .
	manualset3
139091	1	407341	5	NULL	NULL	0	NULL	Specific IgG antibody responses 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific IgG antibody responses in Oestrus ovis L. ( Diptera : Oestridae ) infected sheep : associations with intensity of infection and larval development .
	manualset3
139092	2	407341	5	NULL	NULL	0	NULL	Oestrus ovis L. ( Diptera : Oestridae ) infected sheep	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific IgG antibody responses in Oestrus ovis L. ( Diptera : Oestridae ) infected sheep : associations with intensity of infection and larval development .
	manualset3
139093	3	407341	5	NULL	NULL	0	NULL	associations 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific IgG antibody responses in Oestrus ovis L. ( Diptera : Oestridae ) infected sheep : associations with intensity of infection and larval development .
	manualset3
139094	4	407341	5	NULL	NULL	0	NULL	intensity 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific IgG antibody responses in Oestrus ovis L. ( Diptera : Oestridae ) infected sheep : associations with intensity of infection and larval development .
	manualset3
139095	5	407341	5	NULL	NULL	0	NULL	infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific IgG antibody responses in Oestrus ovis L. ( Diptera : Oestridae ) infected sheep : associations with intensity of infection and larval development .
	manualset3
139096	6	407341	5	NULL	NULL	0	NULL	larval development 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific IgG antibody responses in Oestrus ovis L. ( Diptera : Oestridae ) infected sheep : associations with intensity of infection and larval development .
	manualset3
139097	1	407342	5	NULL	NULL	0	NULL	 NRAS oncogene missense mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific NRAS oncogene missense mutations have been frequently found in some tumors and several hematological diseases , especially in those of myeloid origin .
	manualset3
139098	2	407342	5	NULL	NULL	0	NULL	tumors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific NRAS oncogene missense mutations have been frequently found in some tumors and several hematological diseases , especially in those of myeloid origin .
	manualset3
139099	3	407342	5	NULL	NULL	0	NULL	hematological diseases 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific NRAS oncogene missense mutations have been frequently found in some tumors and several hematological diseases , especially in those of myeloid origin .
	manualset3
139100	4	407342	5	NULL	NULL	0	NULL	myeloid origin	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific NRAS oncogene missense mutations have been frequently found in some tumors and several hematological diseases , especially in those of myeloid origin .
	manualset3
139101	1	407343	5	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific binding of the NADPH-analog , AADP ( + ) , to the FR conformation resulted in dynamic fluorescence quenching in support of the multiple quenching sites model .
	manualset3
139102	2	407343	5	NULL	NULL	0	NULL	NADPH-analog , AADP ( + ) 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific binding of the NADPH-analog , AADP ( + ) , to the FR conformation resulted in dynamic fluorescence quenching in support of the multiple quenching sites model .
	manualset3
139103	3	407343	5	NULL	NULL	0	NULL	FR conformation	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific binding of the NADPH-analog , AADP ( + ) , to the FR conformation resulted in dynamic fluorescence quenching in support of the multiple quenching sites model .
	manualset3
139104	4	407343	5	NULL	NULL	0	NULL	dynamic fluorescence quenching	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific binding of the NADPH-analog , AADP ( + ) , to the FR conformation resulted in dynamic fluorescence quenching in support of the multiple quenching sites model .
	manualset3
139105	5	407343	5	NULL	NULL	0	NULL	multiple quenching sites model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific binding of the NADPH-analog , AADP ( + ) , to the FR conformation resulted in dynamic fluorescence quenching in support of the multiple quenching sites model .
	manualset3
139106	1	407344	5	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific binding was only identified in the kidney consistent with the known distribution of antidiuretic V2 receptors on renal collecting tubules .
	manualset3
139107	2	407344	5	NULL	NULL	0	NULL	kidney 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific binding was only identified in the kidney consistent with the known distribution of antidiuretic V2 receptors on renal collecting tubules .
	manualset3
139108	3	407344	5	NULL	NULL	0	NULL	distribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific binding was only identified in the kidney consistent with the known distribution of antidiuretic V2 receptors on renal collecting tubules .
	manualset3
139109	4	407344	5	NULL	NULL	0	NULL	antidiuretic V2 receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific binding was only identified in the kidney consistent with the known distribution of antidiuretic V2 receptors on renal collecting tubules .
	manualset3
139110	5	407344	5	NULL	NULL	0	NULL	renal collecting tubules	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific binding was only identified in the kidney consistent with the known distribution of antidiuretic V2 receptors on renal collecting tubules .
	manualset3
139111	1	407345	5	NULL	NULL	NULL	NULL	brain protein changes	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Specific brain protein changes correlated with behaviourally effective brain transplants .
	manualset3
139112	2	407345	5	NULL	NULL	0	NULL	behaviourally effective brain transplants 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific brain protein changes correlated with behaviourally effective brain transplants .
	manualset3
139113	1	407346	5	NULL	NULL	0	NULL	cell-cell attachments	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific cell-cell attachments are observed between the living cells in these aggregates .
	manualset3
139114	2	407346	5	NULL	NULL	0	NULL	living cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific cell-cell attachments are observed between the living cells in these aggregates .
	manualset3
139115	3	407346	5	NULL	NULL	0	NULL	aggregates 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific cell-cell attachments are observed between the living cells in these aggregates .
	manualset3
139116	1	407347	5	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A patient with tuberculous meningitis developed a pellagra-like skin eruption after treatment with isoniazid .
	manualset3
139117	2	407347	5	NULL	NULL	0	NULL	tuberculous meningitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A patient with tuberculous meningitis developed a pellagra-like skin eruption after treatment with isoniazid .
	manualset3
139118	3	407347	5	NULL	NULL	0	NULL	pellagra-like skin eruption	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A patient with tuberculous meningitis developed a pellagra-like skin eruption after treatment with isoniazid .
	manualset3
139119	4	407347	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A patient with tuberculous meningitis developed a pellagra-like skin eruption after treatment with isoniazid .
	manualset3
139120	5	407347	5	NULL	NULL	0	NULL	isoniazid 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A patient with tuberculous meningitis developed a pellagra-like skin eruption after treatment with isoniazid .
	manualset3
139121	1	407348	5	NULL	NULL	0	NULL	cross-gender behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific cross-gender behavior in boyhood and later homosexual orientation .
	manualset3
139122	2	407348	5	NULL	NULL	0	NULL	boyhood 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific cross-gender behavior in boyhood and later homosexual orientation .
	manualset3
139123	3	407348	5	NULL	NULL	0	NULL	homosexual orientation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific cross-gender behavior in boyhood and later homosexual orientation .
	manualset3
139124	1	407349	5	NULL	NULL	0	NULL	difficulties 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific difficulties and advantages identified by online faculty were categorized into four broad areas of impact on the teaching/learning experience : ( a ) faculty workload , ( b ) access to education , ( c ) adapting to technology , and ( d ) instructional quality .
	manualset3
139125	2	407349	5	NULL	NULL	0	NULL	advantages 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific difficulties and advantages identified by online faculty were categorized into four broad areas of impact on the teaching/learning experience : ( a ) faculty workload , ( b ) access to education , ( c ) adapting to technology , and ( d ) instructional quality .
	manualset3
139126	3	407349	5	NULL	NULL	0	NULL	online faculty	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific difficulties and advantages identified by online faculty were categorized into four broad areas of impact on the teaching/learning experience : ( a ) faculty workload , ( b ) access to education , ( c ) adapting to technology , and ( d ) instructional quality .
	manualset3
139127	4	407349	5	NULL	NULL	0	NULL	four 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific difficulties and advantages identified by online faculty were categorized into four broad areas of impact on the teaching/learning experience : ( a ) faculty workload , ( b ) access to education , ( c ) adapting to technology , and ( d ) instructional quality .
	manualset3
139128	5	407349	5	NULL	NULL	0	NULL	broad areas	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific difficulties and advantages identified by online faculty were categorized into four broad areas of impact on the teaching/learning experience : ( a ) faculty workload , ( b ) access to education , ( c ) adapting to technology , and ( d ) instructional quality .
	manualset3
139129	6	407349	5	NULL	NULL	0	NULL	impact 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific difficulties and advantages identified by online faculty were categorized into four broad areas of impact on the teaching/learning experience : ( a ) faculty workload , ( b ) access to education , ( c ) adapting to technology , and ( d ) instructional quality .
	manualset3
139130	7	407349	5	NULL	NULL	0	NULL	teaching/learning experience 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific difficulties and advantages identified by online faculty were categorized into four broad areas of impact on the teaching/learning experience : ( a ) faculty workload , ( b ) access to education , ( c ) adapting to technology , and ( d ) instructional quality .
	manualset3
139131	8	407349	5	NULL	NULL	0	NULL	faculty workload	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific difficulties and advantages identified by online faculty were categorized into four broad areas of impact on the teaching/learning experience : ( a ) faculty workload , ( b ) access to education , ( c ) adapting to technology , and ( d ) instructional quality .
	manualset3
139132	9	407349	5	NULL	NULL	0	NULL	education 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific difficulties and advantages identified by online faculty were categorized into four broad areas of impact on the teaching/learning experience : ( a ) faculty workload , ( b ) access to education , ( c ) adapting to technology , and ( d ) instructional quality .
	manualset3
139133	10	407349	5	NULL	NULL	0	NULL	technology 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific difficulties and advantages identified by online faculty were categorized into four broad areas of impact on the teaching/learning experience : ( a ) faculty workload , ( b ) access to education , ( c ) adapting to technology , and ( d ) instructional quality .
	manualset3
139134	11	407349	5	NULL	NULL	0	NULL	instructional quality	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific difficulties and advantages identified by online faculty were categorized into four broad areas of impact on the teaching/learning experience : ( a ) faculty workload , ( b ) access to education , ( c ) adapting to technology , and ( d ) instructional quality .
	manualset3
139135	1	407350	5	NULL	NULL	0	NULL	disruption 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific disruption of the creB gene resulted in similar increased levels of beta-lactamase expression , so it was concluded that CreB represses the transcription of ampH and cepH in a cre ( + ) E. coli strain .
	manualset3
139136	2	407350	5	NULL	NULL	0	NULL	creB gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific disruption of the creB gene resulted in similar increased levels of beta-lactamase expression , so it was concluded that CreB represses the transcription of ampH and cepH in a cre ( + ) E. coli strain .
	manualset3
139137	3	407350	5	NULL	NULL	0	NULL	levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific disruption of the creB gene resulted in similar increased levels of beta-lactamase expression , so it was concluded that CreB represses the transcription of ampH and cepH in a cre ( + ) E. coli strain .
	manualset3
139138	4	407350	5	NULL	NULL	0	NULL	beta-lactamase expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific disruption of the creB gene resulted in similar increased levels of beta-lactamase expression , so it was concluded that CreB represses the transcription of ampH and cepH in a cre ( + ) E. coli strain .
	manualset3
139139	5	407350	5	NULL	NULL	0	NULL	CreB 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific disruption of the creB gene resulted in similar increased levels of beta-lactamase expression , so it was concluded that CreB represses the transcription of ampH and cepH in a cre ( + ) E. coli strain .
	manualset3
139140	6	407350	5	NULL	NULL	0	NULL	transcription 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific disruption of the creB gene resulted in similar increased levels of beta-lactamase expression , so it was concluded that CreB represses the transcription of ampH and cepH in a cre ( + ) E. coli strain .
	manualset3
139141	7	407350	5	NULL	NULL	0	NULL	ampH 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific disruption of the creB gene resulted in similar increased levels of beta-lactamase expression , so it was concluded that CreB represses the transcription of ampH and cepH in a cre ( + ) E. coli strain .
	manualset3
139142	8	407350	5	NULL	NULL	0	NULL	cepH 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific disruption of the creB gene resulted in similar increased levels of beta-lactamase expression , so it was concluded that CreB represses the transcription of ampH and cepH in a cre ( + ) E. coli strain .
	manualset3
139143	9	407350	5	NULL	NULL	0	NULL	cre ( + ) E. coli strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific disruption of the creB gene resulted in similar increased levels of beta-lactamase expression , so it was concluded that CreB represses the transcription of ampH and cepH in a cre ( + ) E. coli strain .
	manualset3
139144	1	407351	5	NULL	NULL	0	NULL	goals 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific goals for the first year of the QT Core were to develop a team of improvement science experts , engage faculty and staff in QT initiatives , promote accountability for excellence in clinical care , and establish specific metrics to evaluate process , structure , and outcomes for QT Core projects .
	manualset3
139145	2	407351	5	NULL	NULL	0	NULL	first year	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific goals for the first year of the QT Core were to develop a team of improvement science experts , engage faculty and staff in QT initiatives , promote accountability for excellence in clinical care , and establish specific metrics to evaluate process , structure , and outcomes for QT Core projects .
	manualset3
139146	3	407351	5	NULL	NULL	0	NULL	QT Core	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific goals for the first year of the QT Core were to develop a team of improvement science experts , engage faculty and staff in QT initiatives , promote accountability for excellence in clinical care , and establish specific metrics to evaluate process , structure , and outcomes for QT Core projects .
	manualset3
139147	4	407351	5	NULL	NULL	0	NULL	team 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific goals for the first year of the QT Core were to develop a team of improvement science experts , engage faculty and staff in QT initiatives , promote accountability for excellence in clinical care , and establish specific metrics to evaluate process , structure , and outcomes for QT Core projects .
	manualset3
139148	5	407351	5	NULL	NULL	0	NULL	science experts	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific goals for the first year of the QT Core were to develop a team of improvement science experts , engage faculty and staff in QT initiatives , promote accountability for excellence in clinical care , and establish specific metrics to evaluate process , structure , and outcomes for QT Core projects .
	manualset3
139149	6	407351	5	NULL	NULL	0	NULL	faculty 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific goals for the first year of the QT Core were to develop a team of improvement science experts , engage faculty and staff in QT initiatives , promote accountability for excellence in clinical care , and establish specific metrics to evaluate process , structure , and outcomes for QT Core projects .
	manualset3
139150	7	407351	5	NULL	NULL	0	NULL	staff 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific goals for the first year of the QT Core were to develop a team of improvement science experts , engage faculty and staff in QT initiatives , promote accountability for excellence in clinical care , and establish specific metrics to evaluate process , structure , and outcomes for QT Core projects .
	manualset3
139151	8	407351	5	NULL	NULL	0	NULL	QT initiatives	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific goals for the first year of the QT Core were to develop a team of improvement science experts , engage faculty and staff in QT initiatives , promote accountability for excellence in clinical care , and establish specific metrics to evaluate process , structure , and outcomes for QT Core projects .
	manualset3
139152	9	407351	5	NULL	NULL	0	NULL	accountability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific goals for the first year of the QT Core were to develop a team of improvement science experts , engage faculty and staff in QT initiatives , promote accountability for excellence in clinical care , and establish specific metrics to evaluate process , structure , and outcomes for QT Core projects .
	manualset3
139153	10	407351	5	NULL	NULL	0	NULL	excellence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific goals for the first year of the QT Core were to develop a team of improvement science experts , engage faculty and staff in QT initiatives , promote accountability for excellence in clinical care , and establish specific metrics to evaluate process , structure , and outcomes for QT Core projects .
	manualset3
139154	11	407351	5	NULL	NULL	0	NULL	clinical care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific goals for the first year of the QT Core were to develop a team of improvement science experts , engage faculty and staff in QT initiatives , promote accountability for excellence in clinical care , and establish specific metrics to evaluate process , structure , and outcomes for QT Core projects .
	manualset3
139155	12	407351	5	NULL	NULL	0	NULL	specific metrics	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific goals for the first year of the QT Core were to develop a team of improvement science experts , engage faculty and staff in QT initiatives , promote accountability for excellence in clinical care , and establish specific metrics to evaluate process , structure , and outcomes for QT Core projects .
	manualset3
139156	13	407351	5	NULL	NULL	0	NULL	process 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific goals for the first year of the QT Core were to develop a team of improvement science experts , engage faculty and staff in QT initiatives , promote accountability for excellence in clinical care , and establish specific metrics to evaluate process , structure , and outcomes for QT Core projects .
	manualset3
139157	14	407351	5	NULL	NULL	0	NULL	structure 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific goals for the first year of the QT Core were to develop a team of improvement science experts , engage faculty and staff in QT initiatives , promote accountability for excellence in clinical care , and establish specific metrics to evaluate process , structure , and outcomes for QT Core projects .
	manualset3
139158	15	407351	5	NULL	NULL	0	NULL	outcomes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific goals for the first year of the QT Core were to develop a team of improvement science experts , engage faculty and staff in QT initiatives , promote accountability for excellence in clinical care , and establish specific metrics to evaluate process , structure , and outcomes for QT Core projects .
	manualset3
139159	16	407351	5	NULL	NULL	0	NULL	QT Core projects	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific goals for the first year of the QT Core were to develop a team of improvement science experts , engage faculty and staff in QT initiatives , promote accountability for excellence in clinical care , and establish specific metrics to evaluate process , structure , and outcomes for QT Core projects .
	manualset3
139160	1	407352	5	NULL	NULL	0	NULL	isotypes 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific isotypes were detected with monoclonal antibodies specific for each human Ig isotype , followed by a peroxidase-conjugated anti-mouse Ig .
	manualset3
139161	2	407352	5	NULL	NULL	0	NULL	monoclonal antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific isotypes were detected with monoclonal antibodies specific for each human Ig isotype , followed by a peroxidase-conjugated anti-mouse Ig .
	manualset3
139162	3	407352	5	NULL	NULL	0	NULL	human Ig isotype	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific isotypes were detected with monoclonal antibodies specific for each human Ig isotype , followed by a peroxidase-conjugated anti-mouse Ig .
	manualset3
139163	4	407352	5	NULL	NULL	0	NULL	peroxidase-conjugated anti-mouse Ig	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific isotypes were detected with monoclonal antibodies specific for each human Ig isotype , followed by a peroxidase-conjugated anti-mouse Ig .
	manualset3
139164	1	407353	5	NULL	NULL	0	NULL	mechanisms 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific mechanisms to orchestrate the growth of the cortex in surface area rather than in thickness are likely to exist , but they have not been identified .
	manualset3
139165	2	407353	5	NULL	NULL	0	NULL	growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific mechanisms to orchestrate the growth of the cortex in surface area rather than in thickness are likely to exist , but they have not been identified .
	manualset3
139166	3	407353	5	NULL	NULL	0	NULL	cortex 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific mechanisms to orchestrate the growth of the cortex in surface area rather than in thickness are likely to exist , but they have not been identified .
	manualset3
139167	4	407353	5	NULL	NULL	0	NULL	surface area 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific mechanisms to orchestrate the growth of the cortex in surface area rather than in thickness are likely to exist , but they have not been identified .
	manualset3
139168	5	407353	5	NULL	NULL	0	NULL	thickness 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific mechanisms to orchestrate the growth of the cortex in surface area rather than in thickness are likely to exist , but they have not been identified .
	manualset3
139169	1	407354	5	NULL	NULL	0	NULL	opioid-amphetamine interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific opioid-amphetamine interactions in the caudate putamen .
	manualset3
139170	2	407354	5	NULL	NULL	0	NULL	caudate putamen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific opioid-amphetamine interactions in the caudate putamen .
	manualset3
139171	1	407355	5	NULL	NULL	0	NULL	phenotypes 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific phenotypes of severe asthma are only beginning to be defined .
	manualset3
139172	2	407355	5	NULL	NULL	0	NULL	severe asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific phenotypes of severe asthma are only beginning to be defined .
	manualset3
139173	1	407356	5	NULL	NULL	0	NULL	pattern 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A pattern of recurrent EEG synchronization was distinguished in all rapid eye movement ( REM ) sleep phases .
	manualset3
139174	2	407356	5	NULL	NULL	0	NULL	recurrent EEG synchronization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A pattern of recurrent EEG synchronization was distinguished in all rapid eye movement ( REM ) sleep phases .
	manualset3
139175	3	407356	5	NULL	NULL	0	NULL	rapid eye movement ( REM ) sleep phases	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A pattern of recurrent EEG synchronization was distinguished in all rapid eye movement ( REM ) sleep phases .
	manualset3
139176	1	407357	5	NULL	NULL	0	NULL	surgical events	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific surgical events can release emboli blocking cerebral arteries and cause catastrophic neurologic sequelae plagueing the patients , their families and the health care system .
	manualset3
139177	2	407357	5	NULL	NULL	0	NULL	emboli blocking cerebral arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific surgical events can release emboli blocking cerebral arteries and cause catastrophic neurologic sequelae plagueing the patients , their families and the health care system .
	manualset3
139178	3	407357	5	NULL	NULL	0	NULL	neurologic sequelae	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific surgical events can release emboli blocking cerebral arteries and cause catastrophic neurologic sequelae plagueing the patients , their families and the health care system .
	manualset3
139179	4	407357	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific surgical events can release emboli blocking cerebral arteries and cause catastrophic neurologic sequelae plagueing the patients , their families and the health care system .
	manualset3
139180	5	407357	5	NULL	NULL	0	NULL	families 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific surgical events can release emboli blocking cerebral arteries and cause catastrophic neurologic sequelae plagueing the patients , their families and the health care system .
	manualset3
139181	6	407357	5	NULL	NULL	0	NULL	health care system	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific surgical events can release emboli blocking cerebral arteries and cause catastrophic neurologic sequelae plagueing the patients , their families and the health care system .
	manualset3
139182	1	407358	5	NULL	NULL	0	NULL	transcription 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific transcription of orthopox virus DNA by HeLa cell RNA polymerase II .
	manualset3
139183	2	407358	5	NULL	NULL	0	NULL	orthopox virus DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific transcription of orthopox virus DNA by HeLa cell RNA polymerase II .
	manualset3
139184	3	407358	5	NULL	NULL	0	NULL	HeLa cell RNA polymerase II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific transcription of orthopox virus DNA by HeLa cell RNA polymerase II .
	manualset3
139185	1	407359	5	NULL	NULL	0	NULL	delay-reduction principle	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , a delay-reduction principle adapted from the conditioned reinforcement literature and a proposed principle of serial stimulus compounds were evaluated against data from delayed matching to sample , serial probe recognition , differential outcome , directed forgetting , and surprisingness preparations .
	manualset3
139186	2	407359	5	NULL	NULL	0	NULL	conditioned reinforcement literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , a delay-reduction principle adapted from the conditioned reinforcement literature and a proposed principle of serial stimulus compounds were evaluated against data from delayed matching to sample , serial probe recognition , differential outcome , directed forgetting , and surprisingness preparations .
	manualset3
139187	3	407359	5	NULL	NULL	0	NULL	principle 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , a delay-reduction principle adapted from the conditioned reinforcement literature and a proposed principle of serial stimulus compounds were evaluated against data from delayed matching to sample , serial probe recognition , differential outcome , directed forgetting , and surprisingness preparations .
	manualset3
139188	4	407359	5	NULL	NULL	0	NULL	serial stimulus compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , a delay-reduction principle adapted from the conditioned reinforcement literature and a proposed principle of serial stimulus compounds were evaluated against data from delayed matching to sample , serial probe recognition , differential outcome , directed forgetting , and surprisingness preparations .
	manualset3
139189	5	407359	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , a delay-reduction principle adapted from the conditioned reinforcement literature and a proposed principle of serial stimulus compounds were evaluated against data from delayed matching to sample , serial probe recognition , differential outcome , directed forgetting , and surprisingness preparations .
	manualset3
139190	6	407359	5	NULL	NULL	0	NULL	sample 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , a delay-reduction principle adapted from the conditioned reinforcement literature and a proposed principle of serial stimulus compounds were evaluated against data from delayed matching to sample , serial probe recognition , differential outcome , directed forgetting , and surprisingness preparations .
	manualset3
139191	7	407359	5	NULL	NULL	0	NULL	serial probe recognition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , a delay-reduction principle adapted from the conditioned reinforcement literature and a proposed principle of serial stimulus compounds were evaluated against data from delayed matching to sample , serial probe recognition , differential outcome , directed forgetting , and surprisingness preparations .
	manualset3
139192	8	407359	5	NULL	NULL	0	NULL	differential outcome	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , a delay-reduction principle adapted from the conditioned reinforcement literature and a proposed principle of serial stimulus compounds were evaluated against data from delayed matching to sample , serial probe recognition , differential outcome , directed forgetting , and surprisingness preparations .
	manualset3
139193	9	407359	5	NULL	NULL	0	NULL	directed forgetting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , a delay-reduction principle adapted from the conditioned reinforcement literature and a proposed principle of serial stimulus compounds were evaluated against data from delayed matching to sample , serial probe recognition , differential outcome , directed forgetting , and surprisingness preparations .
	manualset3
139194	10	407359	5	NULL	NULL	0	NULL	surprisingness preparations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , a delay-reduction principle adapted from the conditioned reinforcement literature and a proposed principle of serial stimulus compounds were evaluated against data from delayed matching to sample , serial probe recognition , differential outcome , directed forgetting , and surprisingness preparations .
	manualset3
139195	1	407360	5	NULL	NULL	0	NULL	apoE	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , apoE induced the phosphorylation of Akt , peaking at 30 min , and the increased phosphorylation of Akt was significantly attenuated after pretreatment with LY294002 ( 50 M ) , an inhibitor of the PI3K signaling pathway .
	manualset3
139196	2	407360	5	NULL	NULL	0	NULL	phosphorylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , apoE induced the phosphorylation of Akt , peaking at 30 min , and the increased phosphorylation of Akt was significantly attenuated after pretreatment with LY294002 ( 50 M ) , an inhibitor of the PI3K signaling pathway .
	manualset3
139197	3	407360	5	NULL	NULL	0	NULL	Akt 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , apoE induced the phosphorylation of Akt , peaking at 30 min , and the increased phosphorylation of Akt was significantly attenuated after pretreatment with LY294002 ( 50 M ) , an inhibitor of the PI3K signaling pathway .
	manualset3
139198	4	407360	5	NULL	NULL	0	NULL	30 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , apoE induced the phosphorylation of Akt , peaking at 30 min , and the increased phosphorylation of Akt was significantly attenuated after pretreatment with LY294002 ( 50 M ) , an inhibitor of the PI3K signaling pathway .
	manualset3
139199	5	407360	5	NULL	NULL	0	NULL	phosphorylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , apoE induced the phosphorylation of Akt , peaking at 30 min , and the increased phosphorylation of Akt was significantly attenuated after pretreatment with LY294002 ( 50 M ) , an inhibitor of the PI3K signaling pathway .
	manualset3
139200	6	407360	5	NULL	NULL	0	NULL	Akt 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , apoE induced the phosphorylation of Akt , peaking at 30 min , and the increased phosphorylation of Akt was significantly attenuated after pretreatment with LY294002 ( 50 M ) , an inhibitor of the PI3K signaling pathway .
	manualset3
139201	7	407360	5	NULL	NULL	0	NULL	pretreatment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , apoE induced the phosphorylation of Akt , peaking at 30 min , and the increased phosphorylation of Akt was significantly attenuated after pretreatment with LY294002 ( 50 M ) , an inhibitor of the PI3K signaling pathway .
	manualset3
139202	8	407360	5	NULL	NULL	0	NULL	LY294002 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , apoE induced the phosphorylation of Akt , peaking at 30 min , and the increased phosphorylation of Akt was significantly attenuated after pretreatment with LY294002 ( 50 M ) , an inhibitor of the PI3K signaling pathway .
	manualset3
139203	9	407360	5	NULL	NULL	0	NULL	50 M 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , apoE induced the phosphorylation of Akt , peaking at 30 min , and the increased phosphorylation of Akt was significantly attenuated after pretreatment with LY294002 ( 50 M ) , an inhibitor of the PI3K signaling pathway .
	manualset3
139204	10	407360	5	NULL	NULL	0	NULL	inhibitor 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , apoE induced the phosphorylation of Akt , peaking at 30 min , and the increased phosphorylation of Akt was significantly attenuated after pretreatment with LY294002 ( 50 M ) , an inhibitor of the PI3K signaling pathway .
	manualset3
139205	11	407360	5	NULL	NULL	0	NULL	PI3K signaling pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , apoE induced the phosphorylation of Akt , peaking at 30 min , and the increased phosphorylation of Akt was significantly attenuated after pretreatment with LY294002 ( 50 M ) , an inhibitor of the PI3K signaling pathway .
	manualset3
139206	1	407361	5	NULL	NULL	0	NULL	receptor signalling 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , does receptor signalling occur only at the plasma membrane ; is signalling dependent upon the location of defined endosome populations ; or are components of both plasma membrane and endosomal activity operative depending upon the particular signalling pathway or cell type ?
	manualset3
139207	2	407361	5	NULL	NULL	0	NULL	plasma membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , does receptor signalling occur only at the plasma membrane ; is signalling dependent upon the location of defined endosome populations ; or are components of both plasma membrane and endosomal activity operative depending upon the particular signalling pathway or cell type ?
	manualset3
139208	3	407361	5	NULL	NULL	0	NULL	location 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , does receptor signalling occur only at the plasma membrane ; is signalling dependent upon the location of defined endosome populations ; or are components of both plasma membrane and endosomal activity operative depending upon the particular signalling pathway or cell type ?
	manualset3
139209	4	407361	5	NULL	NULL	0	NULL	endosome populations	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , does receptor signalling occur only at the plasma membrane ; is signalling dependent upon the location of defined endosome populations ; or are components of both plasma membrane and endosomal activity operative depending upon the particular signalling pathway or cell type ?
	manualset3
139210	5	407361	5	NULL	NULL	0	NULL	components 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , does receptor signalling occur only at the plasma membrane ; is signalling dependent upon the location of defined endosome populations ; or are components of both plasma membrane and endosomal activity operative depending upon the particular signalling pathway or cell type ?
	manualset3
139211	6	407361	5	NULL	NULL	0	NULL	plasma membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , does receptor signalling occur only at the plasma membrane ; is signalling dependent upon the location of defined endosome populations ; or are components of both plasma membrane and endosomal activity operative depending upon the particular signalling pathway or cell type ?
	manualset3
139212	7	407361	5	NULL	NULL	0	NULL	endosomal activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , does receptor signalling occur only at the plasma membrane ; is signalling dependent upon the location of defined endosome populations ; or are components of both plasma membrane and endosomal activity operative depending upon the particular signalling pathway or cell type ?
	manualset3
139213	8	407361	5	NULL	NULL	0	NULL	signalling pathway 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , does receptor signalling occur only at the plasma membrane ; is signalling dependent upon the location of defined endosome populations ; or are components of both plasma membrane and endosomal activity operative depending upon the particular signalling pathway or cell type ?
	manualset3
139214	9	407361	5	NULL	NULL	0	NULL	cell type	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , does receptor signalling occur only at the plasma membrane ; is signalling dependent upon the location of defined endosome populations ; or are components of both plasma membrane and endosomal activity operative depending upon the particular signalling pathway or cell type ?
	manualset3
139215	1	407362	5	NULL	NULL	0	NULL	T lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , invading T lymphocytes contributed to neuronal cell death via the Fas/FasL pathway .
	manualset3
139216	2	407362	5	NULL	NULL	0	NULL	neuronal cell death 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , invading T lymphocytes contributed to neuronal cell death via the Fas/FasL pathway .
	manualset3
139217	3	407362	5	NULL	NULL	0	NULL	Fas/FasL pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , invading T lymphocytes contributed to neuronal cell death via the Fas/FasL pathway .
	manualset3
139218	1	407363	5	NULL	NULL	NULL	NULL	procedure 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Specifically , is it advisable for the procedure to be performed while the woman is still on the delivery table ?
	manualset3
139219	2	407363	5	NULL	NULL	0	NULL	woman 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , is it advisable for the procedure to be performed while the woman is still on the delivery table ?
	manualset3
139220	3	407363	5	NULL	NULL	0	NULL	delivery table	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , is it advisable for the procedure to be performed while the woman is still on the delivery table ?
	manualset3
139221	1	407364	5	NULL	NULL	0	NULL	platelet-derived growth factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , platelet-derived growth factor , neuregulin , and insulin-like growth factor-I all are classified as ligands for receptor-type tyrosine kinase and activate common intracellular signaling cascades , mitogen-activated protein kinase pathways , and phosphatidylinositol-3-kinase pathways .
	manualset3
139222	2	407364	5	NULL	NULL	0	NULL	neuregulin 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , platelet-derived growth factor , neuregulin , and insulin-like growth factor-I all are classified as ligands for receptor-type tyrosine kinase and activate common intracellular signaling cascades , mitogen-activated protein kinase pathways , and phosphatidylinositol-3-kinase pathways .
	manualset3
139223	3	407364	5	NULL	NULL	0	NULL	insulin-like growth factor-I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , platelet-derived growth factor , neuregulin , and insulin-like growth factor-I all are classified as ligands for receptor-type tyrosine kinase and activate common intracellular signaling cascades , mitogen-activated protein kinase pathways , and phosphatidylinositol-3-kinase pathways .
	manualset3
139224	4	407364	5	NULL	NULL	0	NULL	ligands 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , platelet-derived growth factor , neuregulin , and insulin-like growth factor-I all are classified as ligands for receptor-type tyrosine kinase and activate common intracellular signaling cascades , mitogen-activated protein kinase pathways , and phosphatidylinositol-3-kinase pathways .
	manualset3
139225	5	407364	5	NULL	NULL	0	NULL	receptor-type tyrosine kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , platelet-derived growth factor , neuregulin , and insulin-like growth factor-I all are classified as ligands for receptor-type tyrosine kinase and activate common intracellular signaling cascades , mitogen-activated protein kinase pathways , and phosphatidylinositol-3-kinase pathways .
	manualset3
139226	6	407364	5	NULL	NULL	0	NULL	intracellular signaling cascades	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , platelet-derived growth factor , neuregulin , and insulin-like growth factor-I all are classified as ligands for receptor-type tyrosine kinase and activate common intracellular signaling cascades , mitogen-activated protein kinase pathways , and phosphatidylinositol-3-kinase pathways .
	manualset3
139227	7	407364	5	NULL	NULL	0	NULL	mitogen-activated protein kinase pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , platelet-derived growth factor , neuregulin , and insulin-like growth factor-I all are classified as ligands for receptor-type tyrosine kinase and activate common intracellular signaling cascades , mitogen-activated protein kinase pathways , and phosphatidylinositol-3-kinase pathways .
	manualset3
139228	8	407364	5	NULL	NULL	0	NULL	phosphatidylinositol-3-kinase pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , platelet-derived growth factor , neuregulin , and insulin-like growth factor-I all are classified as ligands for receptor-type tyrosine kinase and activate common intracellular signaling cascades , mitogen-activated protein kinase pathways , and phosphatidylinositol-3-kinase pathways .
	manualset3
139229	1	407365	5	NULL	NULL	0	NULL	abnormality 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A peculiar abnormality of the precentral cerebellar vein seen only in cystic astrocytoma of the vermis is reported .
	manualset3
139230	2	407365	5	NULL	NULL	0	NULL	precentral cerebellar vein 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A peculiar abnormality of the precentral cerebellar vein seen only in cystic astrocytoma of the vermis is reported .
	manualset3
139231	3	407365	5	NULL	NULL	0	NULL	cystic astrocytoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A peculiar abnormality of the precentral cerebellar vein seen only in cystic astrocytoma of the vermis is reported .
	manualset3
139232	4	407365	5	NULL	NULL	0	NULL	vermis 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A peculiar abnormality of the precentral cerebellar vein seen only in cystic astrocytoma of the vermis is reported .
	manualset3
139233	1	407366	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , this study investigated the relations among three religious orientations ( intrinsic , extrinsic-personal , and extrinsic-social ) and job involvement for 100 employees of a rehabilitation hospital in the southern United States .
	manualset3
139234	2	407366	5	NULL	NULL	0	NULL	relations 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , this study investigated the relations among three religious orientations ( intrinsic , extrinsic-personal , and extrinsic-social ) and job involvement for 100 employees of a rehabilitation hospital in the southern United States .
	manualset3
139235	3	407366	5	NULL	NULL	0	NULL	three 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , this study investigated the relations among three religious orientations ( intrinsic , extrinsic-personal , and extrinsic-social ) and job involvement for 100 employees of a rehabilitation hospital in the southern United States .
	manualset3
139236	4	407366	5	NULL	NULL	0	NULL	religious orientations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , this study investigated the relations among three religious orientations ( intrinsic , extrinsic-personal , and extrinsic-social ) and job involvement for 100 employees of a rehabilitation hospital in the southern United States .
	manualset3
139237	5	407366	5	NULL	NULL	0	NULL	job involvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , this study investigated the relations among three religious orientations ( intrinsic , extrinsic-personal , and extrinsic-social ) and job involvement for 100 employees of a rehabilitation hospital in the southern United States .
	manualset3
139238	6	407366	5	NULL	NULL	0	NULL	100 employees	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , this study investigated the relations among three religious orientations ( intrinsic , extrinsic-personal , and extrinsic-social ) and job involvement for 100 employees of a rehabilitation hospital in the southern United States .
	manualset3
139239	7	407366	5	NULL	NULL	0	NULL	rehabilitation hospital	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , this study investigated the relations among three religious orientations ( intrinsic , extrinsic-personal , and extrinsic-social ) and job involvement for 100 employees of a rehabilitation hospital in the southern United States .
	manualset3
139240	8	407366	5	NULL	NULL	0	NULL	southern United States	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , this study investigated the relations among three religious orientations ( intrinsic , extrinsic-personal , and extrinsic-social ) and job involvement for 100 employees of a rehabilitation hospital in the southern United States .
	manualset3
139241	1	407367	5	NULL	NULL	0	NULL	cofilin , an actin destabilizing protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , we employ cofilin , an actin destabilizing protein that binds and severs filaments , and phalloidin , a fungal toxin that binds and stabilizes F-actin .
	manualset3
139242	2	407367	5	NULL	NULL	0	NULL	filaments 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , we employ cofilin , an actin destabilizing protein that binds and severs filaments , and phalloidin , a fungal toxin that binds and stabilizes F-actin .
	manualset3
139243	3	407367	5	NULL	NULL	0	NULL	phalloidin , a fungal toxin	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , we employ cofilin , an actin destabilizing protein that binds and severs filaments , and phalloidin , a fungal toxin that binds and stabilizes F-actin .
	manualset3
139244	4	407367	5	NULL	NULL	0	NULL	F-actin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , we employ cofilin , an actin destabilizing protein that binds and severs filaments , and phalloidin , a fungal toxin that binds and stabilizes F-actin .
	manualset3
139245	1	407368	5	NULL	NULL	0	NULL	research findings 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , we review research findings showing that attachment insecurity is a major contributor to mental disorders , and that the enhancement of attachment security can facilitate amelioration of psychopathology .
	manualset3
139246	2	407368	5	NULL	NULL	0	NULL	attachment insecurity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , we review research findings showing that attachment insecurity is a major contributor to mental disorders , and that the enhancement of attachment security can facilitate amelioration of psychopathology .
	manualset3
139247	3	407368	5	NULL	NULL	0	NULL	major contributor 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , we review research findings showing that attachment insecurity is a major contributor to mental disorders , and that the enhancement of attachment security can facilitate amelioration of psychopathology .
	manualset3
139248	4	407368	5	NULL	NULL	0	NULL	mental disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , we review research findings showing that attachment insecurity is a major contributor to mental disorders , and that the enhancement of attachment security can facilitate amelioration of psychopathology .
	manualset3
139249	5	407368	5	NULL	NULL	0	NULL	enhancement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , we review research findings showing that attachment insecurity is a major contributor to mental disorders , and that the enhancement of attachment security can facilitate amelioration of psychopathology .
	manualset3
139250	6	407368	5	NULL	NULL	0	NULL	attachment security 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , we review research findings showing that attachment insecurity is a major contributor to mental disorders , and that the enhancement of attachment security can facilitate amelioration of psychopathology .
	manualset3
139251	7	407368	5	NULL	NULL	0	NULL	amelioration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , we review research findings showing that attachment insecurity is a major contributor to mental disorders , and that the enhancement of attachment security can facilitate amelioration of psychopathology .
	manualset3
139252	8	407368	5	NULL	NULL	0	NULL	psychopathology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , we review research findings showing that attachment insecurity is a major contributor to mental disorders , and that the enhancement of attachment security can facilitate amelioration of psychopathology .
	manualset3
139253	1	407369	5	NULL	NULL	0	NULL	IncF plasmid conjugation genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Specificities of IncF plasmid conjugation genes .
	manualset3
142885	2	407369	5	NULL	NULL	0	NULL	Specificities 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specificities of IncF plasmid conjugation genes .
	manualset3
139254	1	407370	5	NULL	NULL	0	NULL	Specificity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specificity and cross-reactivity of monoclonal antibodies reactive with the core and lipid A regions of bacterial lipopolysaccharide .
	manualset3
139255	2	407370	5	NULL	NULL	0	NULL	cross-reactivity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Specificity and cross-reactivity of monoclonal antibodies reactive with the core and lipid A regions of bacterial lipopolysaccharide .
	manualset3
139256	3	407370	5	NULL	NULL	0	NULL	monoclonal antibodies 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Specificity and cross-reactivity of monoclonal antibodies reactive with the core and lipid A regions of bacterial lipopolysaccharide .
	manualset3
139257	4	407370	5	NULL	NULL	0	NULL	core regions 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Specificity and cross-reactivity of monoclonal antibodies reactive with the core and lipid A regions of bacterial lipopolysaccharide .
	manualset3
139258	5	407370	5	NULL	NULL	0	NULL	lipid A regions 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Specificity and cross-reactivity of monoclonal antibodies reactive with the core and lipid A regions of bacterial lipopolysaccharide .
	manualset3
139259	6	407370	5	NULL	NULL	0	NULL	bacterial lipopolysaccharide	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Specificity and cross-reactivity of monoclonal antibodies reactive with the core and lipid A regions of bacterial lipopolysaccharide .
	manualset3
139260	1	407371	5	NULL	NULL	0	NULL	Specificity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specificity of oligodeoxynucleotide binding of mouse uterine cytosol estradiol receptors .
	manualset3
139261	2	407371	5	NULL	NULL	0	NULL	oligodeoxynucleotide binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Specificity of oligodeoxynucleotide binding of mouse uterine cytosol estradiol receptors .
	manualset3
139262	3	407371	5	NULL	NULL	0	NULL	mouse uterine cytosol estradiol receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Specificity of oligodeoxynucleotide binding of mouse uterine cytosol estradiol receptors .
	manualset3
139263	1	407372	5	NULL	NULL	0	NULL	Specificity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specificity of this test was examined by an inhibition test using ss-DNA and double-stranded DNA ( ds-DNA ) .
	manualset3
139264	2	407372	5	NULL	NULL	NULL	NULL	test 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Specificity of this test was examined by an inhibition test using ss-DNA and double-stranded DNA ( ds-DNA ) .
	manualset3
139265	3	407372	5	NULL	NULL	0	NULL	inhibition test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Specificity of this test was examined by an inhibition test using ss-DNA and double-stranded DNA ( ds-DNA ) .
	manualset3
139266	4	407372	5	NULL	NULL	0	NULL	ss-DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Specificity of this test was examined by an inhibition test using ss-DNA and double-stranded DNA ( ds-DNA ) .
	manualset3
139267	5	407372	5	NULL	NULL	0	NULL	double-stranded DNA ( ds-DNA )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Specificity of this test was examined by an inhibition test using ss-DNA and double-stranded DNA ( ds-DNA ) .
	manualset3
139268	1	407373	5	NULL	NULL	0	NULL	Specimens 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Specimens of the spleen from animals with implants showed light 3-10-microns structures that were not observed in those without implants .
	manualset3
139269	2	407373	5	NULL	NULL	0	NULL	spleen 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Specimens of the spleen from animals with implants showed light 3-10-microns structures that were not observed in those without implants .
	manualset3
139270	3	407373	5	NULL	NULL	0	NULL	animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Specimens of the spleen from animals with implants showed light 3-10-microns structures that were not observed in those without implants .
	manualset3
139271	4	407373	5	NULL	NULL	0	NULL	implants 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Specimens of the spleen from animals with implants showed light 3-10-microns structures that were not observed in those without implants .
	manualset3
139272	5	407373	5	NULL	NULL	0	NULL	light 3-10-microns structures	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Specimens of the spleen from animals with implants showed light 3-10-microns structures that were not observed in those without implants .
	manualset3
139273	6	407373	5	NULL	NULL	0	NULL	implants 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Specimens of the spleen from animals with implants showed light 3-10-microns structures that were not observed in those without implants .
	manualset3
139274	1	407374	5	NULL	NULL	0	NULL	peculiar characteristic	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A peculiar characteristic of ASR is its content of nitrogen .
	manualset3
139275	2	407374	5	NULL	NULL	0	NULL	ASR 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A peculiar characteristic of ASR is its content of nitrogen .
	manualset3
139276	3	407374	5	NULL	NULL	0	NULL	content 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A peculiar characteristic of ASR is its content of nitrogen .
	manualset3
139277	4	407374	5	NULL	NULL	0	NULL	nitrogen 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	A peculiar characteristic of ASR is its content of nitrogen .
	manualset3
139278	1	407375	5	NULL	NULL	0	NULL	Spectra 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectra were obtained from fully hydrated samples regenerated with retinals 13C labeled at positions C-5 , C-6 , C-7 , C-8 , and C-18 and from lyophilized samples regenerated with retinals labeled at C-9 and C-13 .
	manualset3
139279	2	407375	5	NULL	NULL	0	NULL	fully hydrated samples	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectra were obtained from fully hydrated samples regenerated with retinals 13C labeled at positions C-5 , C-6 , C-7 , C-8 , and C-18 and from lyophilized samples regenerated with retinals labeled at C-9 and C-13 .
	manualset3
139280	3	407375	5	NULL	NULL	0	NULL	retinals 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectra were obtained from fully hydrated samples regenerated with retinals 13C labeled at positions C-5 , C-6 , C-7 , C-8 , and C-18 and from lyophilized samples regenerated with retinals labeled at C-9 and C-13 .
	manualset3
139281	4	407375	5	NULL	NULL	NULL	NULL	C-5 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Spectra were obtained from fully hydrated samples regenerated with retinals 13C labeled at positions C-5 , C-6 , C-7 , C-8 , and C-18 and from lyophilized samples regenerated with retinals labeled at C-9 and C-13 .
	manualset3
139282	5	407375	5	NULL	NULL	0	NULL	C-6	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectra were obtained from fully hydrated samples regenerated with retinals 13C labeled at positions C-5 , C-6 , C-7 , C-8 , and C-18 and from lyophilized samples regenerated with retinals labeled at C-9 and C-13 .
	manualset3
139283	6	407375	5	NULL	NULL	0	NULL	C-7	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectra were obtained from fully hydrated samples regenerated with retinals 13C labeled at positions C-5 , C-6 , C-7 , C-8 , and C-18 and from lyophilized samples regenerated with retinals labeled at C-9 and C-13 .
	manualset3
139284	7	407375	5	NULL	NULL	0	NULL	C-8	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectra were obtained from fully hydrated samples regenerated with retinals 13C labeled at positions C-5 , C-6 , C-7 , C-8 , and C-18 and from lyophilized samples regenerated with retinals labeled at C-9 and C-13 .
	manualset3
139285	8	407375	5	NULL	NULL	0	NULL	C-18	n												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectra were obtained from fully hydrated samples regenerated with retinals 13C labeled at positions C-5 , C-6 , C-7 , C-8 , and C-18 and from lyophilized samples regenerated with retinals labeled at C-9 and C-13 .
	manualset3
139286	9	407375	5	NULL	NULL	0	NULL	lyophilized samples 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectra were obtained from fully hydrated samples regenerated with retinals 13C labeled at positions C-5 , C-6 , C-7 , C-8 , and C-18 and from lyophilized samples regenerated with retinals labeled at C-9 and C-13 .
	manualset3
139287	10	407375	5	NULL	NULL	0	NULL	retinals 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectra were obtained from fully hydrated samples regenerated with retinals 13C labeled at positions C-5 , C-6 , C-7 , C-8 , and C-18 and from lyophilized samples regenerated with retinals labeled at C-9 and C-13 .
	manualset3
139288	11	407375	5	NULL	NULL	0	NULL	C-9	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectra were obtained from fully hydrated samples regenerated with retinals 13C labeled at positions C-5 , C-6 , C-7 , C-8 , and C-18 and from lyophilized samples regenerated with retinals labeled at C-9 and C-13 .
	manualset3
139289	12	407375	5	NULL	NULL	0	NULL	C-13	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectra were obtained from fully hydrated samples regenerated with retinals 13C labeled at positions C-5 , C-6 , C-7 , C-8 , and C-18 and from lyophilized samples regenerated with retinals labeled at C-9 and C-13 .
	manualset3
139290	1	407376	5	NULL	NULL	0	NULL	Spectra 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectra were simulated by variation of order parameter describing the average amplitude of motion of the long molecular axis of the nitrogen 2 p pi orbital of the spin label and of the respective correlation times .
	manualset3
139291	2	407376	5	NULL	NULL	0	NULL	variation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectra were simulated by variation of order parameter describing the average amplitude of motion of the long molecular axis of the nitrogen 2 p pi orbital of the spin label and of the respective correlation times .
	manualset3
139292	3	407376	5	NULL	NULL	0	NULL	order parameter	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectra were simulated by variation of order parameter describing the average amplitude of motion of the long molecular axis of the nitrogen 2 p pi orbital of the spin label and of the respective correlation times .
	manualset3
139293	4	407376	5	NULL	NULL	0	NULL	average amplitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectra were simulated by variation of order parameter describing the average amplitude of motion of the long molecular axis of the nitrogen 2 p pi orbital of the spin label and of the respective correlation times .
	manualset3
139294	5	407376	5	NULL	NULL	0	NULL	motion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectra were simulated by variation of order parameter describing the average amplitude of motion of the long molecular axis of the nitrogen 2 p pi orbital of the spin label and of the respective correlation times .
	manualset3
139295	6	407376	5	NULL	NULL	0	NULL	long molecular axis 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectra were simulated by variation of order parameter describing the average amplitude of motion of the long molecular axis of the nitrogen 2 p pi orbital of the spin label and of the respective correlation times .
	manualset3
139296	7	407376	5	NULL	NULL	0	NULL	nitrogen 2 p pi orbital 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectra were simulated by variation of order parameter describing the average amplitude of motion of the long molecular axis of the nitrogen 2 p pi orbital of the spin label and of the respective correlation times .
	manualset3
139297	8	407376	5	NULL	NULL	0	NULL	spin label 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectra were simulated by variation of order parameter describing the average amplitude of motion of the long molecular axis of the nitrogen 2 p pi orbital of the spin label and of the respective correlation times .
	manualset3
139298	9	407376	5	NULL	NULL	0	NULL	correlation times 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectra were simulated by variation of order parameter describing the average amplitude of motion of the long molecular axis of the nitrogen 2 p pi orbital of the spin label and of the respective correlation times .
	manualset3
139299	1	407377	5	NULL	NULL	0	NULL	Spectral analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectral analysis of R-R and arterial pressure variabilities to assess sympatho-vagal interaction during mental stress in humans .
	manualset3
139300	2	407377	5	NULL	NULL	0	NULL	 R-R 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectral analysis of R-R and arterial pressure variabilities to assess sympatho-vagal interaction during mental stress in humans .
	manualset3
139301	3	407377	5	NULL	NULL	0	NULL	arterial pressure variabilities	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectral analysis of R-R and arterial pressure variabilities to assess sympatho-vagal interaction during mental stress in humans .
	manualset3
139302	4	407377	5	NULL	NULL	0	NULL	sympatho-vagal interaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectral analysis of R-R and arterial pressure variabilities to assess sympatho-vagal interaction during mental stress in humans .
	manualset3
139303	5	407377	5	NULL	NULL	0	NULL	mental stress 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectral analysis of R-R and arterial pressure variabilities to assess sympatho-vagal interaction during mental stress in humans .
	manualset3
139304	6	407377	5	NULL	NULL	0	NULL	humans 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectral analysis of R-R and arterial pressure variabilities to assess sympatho-vagal interaction during mental stress in humans .
	manualset3
139305	1	407378	5	NULL	NULL	0	NULL	Spectral identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectral identification of fullerene C82 isomers .
	manualset3
139306	2	407378	5	NULL	NULL	0	NULL	fullerene C82 isomers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectral identification of fullerene C82 isomers .
	manualset3
139307	1	407379	5	NULL	NULL	0	NULL	Spectrophotometric determination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectrophotometric determination of microgram quantities of protein without nucleic acid interference .
	manualset3
139308	2	407379	5	NULL	NULL	0	NULL	microgram quantities	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectrophotometric determination of microgram quantities of protein without nucleic acid interference .
	manualset3
139309	3	407379	5	NULL	NULL	0	NULL	protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectrophotometric determination of microgram quantities of protein without nucleic acid interference .
	manualset3
139310	4	407379	5	NULL	NULL	0	NULL	nucleic acid interference 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectrophotometric determination of microgram quantities of protein without nucleic acid interference .
	manualset3
139311	1	407380	5	NULL	NULL	0	NULL	Spectroscopic investigations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectroscopic investigations of new binuclear transition metal complexes of Schiff bases derived from 4 , 6-diacetylresorcinol and 3-amino-1-propanol or 1 , 3-diamino-propane .
	manualset3
139312	2	407380	5	NULL	NULL	0	NULL	binuclear transition metal complexes	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectroscopic investigations of new binuclear transition metal complexes of Schiff bases derived from 4 , 6-diacetylresorcinol and 3-amino-1-propanol or 1 , 3-diamino-propane .
	manualset3
139313	3	407380	5	NULL	NULL	0	NULL	Schiff bases derived from 4 , 6-diacetylresorcinol and 3-amino-1-propanol or 1 , 3-diamino-propane	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectroscopic investigations of new binuclear transition metal complexes of Schiff bases derived from 4 , 6-diacetylresorcinol and 3-amino-1-propanol or 1 , 3-diamino-propane .
	manualset3
139314	1	407381	5	NULL	NULL	0	NULL	Spectroscopic studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectroscopic studies and life time measurements of binding of a bioactive compound to bovine serum albumin and the effects of common ions and other drugs on binding .
	manualset3
139315	2	407381	5	NULL	NULL	0	NULL	life time measurements	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectroscopic studies and life time measurements of binding of a bioactive compound to bovine serum albumin and the effects of common ions and other drugs on binding .
	manualset3
139316	3	407381	5	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectroscopic studies and life time measurements of binding of a bioactive compound to bovine serum albumin and the effects of common ions and other drugs on binding .
	manualset3
139317	4	407381	5	NULL	NULL	0	NULL	bioactive compound 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectroscopic studies and life time measurements of binding of a bioactive compound to bovine serum albumin and the effects of common ions and other drugs on binding .
	manualset3
139318	5	407381	5	NULL	NULL	0	NULL	bovine serum albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectroscopic studies and life time measurements of binding of a bioactive compound to bovine serum albumin and the effects of common ions and other drugs on binding .
	manualset3
139319	6	407381	5	NULL	NULL	0	NULL	common ions 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectroscopic studies and life time measurements of binding of a bioactive compound to bovine serum albumin and the effects of common ions and other drugs on binding .
	manualset3
139320	7	407381	5	NULL	NULL	0	NULL	drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectroscopic studies and life time measurements of binding of a bioactive compound to bovine serum albumin and the effects of common ions and other drugs on binding .
	manualset3
139321	8	407381	5	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectroscopic studies and life time measurements of binding of a bioactive compound to bovine serum albumin and the effects of common ions and other drugs on binding .
	manualset3
139692	9	407381	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectroscopic studies and life time measurements of binding of a bioactive compound to bovine serum albumin and the effects of common ions and other drugs on binding .
	manualset3
139322	1	407382	5	NULL	NULL	0	NULL	Spectroscopic studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectroscopic studies of interactions between C.I. Reactive Orange 16 with alkyltrimethylammonium bromide surfactants .
	manualset3
139323	2	407382	5	NULL	NULL	0	NULL	interactions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectroscopic studies of interactions between C.I. Reactive Orange 16 with alkyltrimethylammonium bromide surfactants .
	manualset3
139324	3	407382	5	NULL	NULL	0	NULL	C.I. Reactive Orange 16 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectroscopic studies of interactions between C.I. Reactive Orange 16 with alkyltrimethylammonium bromide surfactants .
	manualset3
139325	4	407382	5	NULL	NULL	0	NULL	alkyltrimethylammonium bromide surfactants	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Spectroscopic studies of interactions between C.I. Reactive Orange 16 with alkyltrimethylammonium bromide surfactants .
	manualset3
139326	1	407383	5	NULL	NULL	0	NULL	minimally invasive cardiac surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A peril of minimally invasive cardiac surgery .
	manualset3
139327	1	407384	5	NULL	NULL	0	NULL	Sperm chromatin abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sperm chromatin abnormalities were measured flow cytometrically according to the Sperm Chromatin Structure Assay method : after chromatin denaturation by low pH , sperm cells were stained with metachromatic fluorochrome acridine orange .
	manualset3
139328	2	407384	5	NULL	NULL	0	NULL	Sperm Chromatin Structure Assay method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sperm chromatin abnormalities were measured flow cytometrically according to the Sperm Chromatin Structure Assay method : after chromatin denaturation by low pH , sperm cells were stained with metachromatic fluorochrome acridine orange .
	manualset3
139329	3	407384	5	NULL	NULL	0	NULL	chromatin denaturation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sperm chromatin abnormalities were measured flow cytometrically according to the Sperm Chromatin Structure Assay method : after chromatin denaturation by low pH , sperm cells were stained with metachromatic fluorochrome acridine orange .
	manualset3
139330	4	407384	5	NULL	NULL	0	NULL	low pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sperm chromatin abnormalities were measured flow cytometrically according to the Sperm Chromatin Structure Assay method : after chromatin denaturation by low pH , sperm cells were stained with metachromatic fluorochrome acridine orange .
	manualset3
139331	5	407384	5	NULL	NULL	0	NULL	sperm cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Sperm chromatin abnormalities were measured flow cytometrically according to the Sperm Chromatin Structure Assay method : after chromatin denaturation by low pH , sperm cells were stained with metachromatic fluorochrome acridine orange .
	manualset3
139332	6	407384	5	NULL	NULL	0	NULL	metachromatic fluorochrome acridine orange	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Sperm chromatin abnormalities were measured flow cytometrically according to the Sperm Chromatin Structure Assay method : after chromatin denaturation by low pH , sperm cells were stained with metachromatic fluorochrome acridine orange .
	manualset3
139333	1	407385	5	NULL	NULL	0	NULL	Spermatogonial stem cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Spermatogonial stem cells from a fertile donor can be transplanted to the testes of infertile recipients and generate sperm .
	manualset3
139334	2	407385	5	NULL	NULL	0	NULL	fertile donor	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Spermatogonial stem cells from a fertile donor can be transplanted to the testes of infertile recipients and generate sperm .
	manualset3
139335	3	407385	5	NULL	NULL	0	NULL	testes 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Spermatogonial stem cells from a fertile donor can be transplanted to the testes of infertile recipients and generate sperm .
	manualset3
139336	4	407385	5	NULL	NULL	0	NULL	infertile recipients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Spermatogonial stem cells from a fertile donor can be transplanted to the testes of infertile recipients and generate sperm .
	manualset3
139337	5	407385	5	NULL	NULL	0	NULL	sperm 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Spermatogonial stem cells from a fertile donor can be transplanted to the testes of infertile recipients and generate sperm .
	manualset3
139338	1	407386	5	NULL	NULL	0	NULL	Spermatozoa 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Spermatozoa , both normal ( acrosome-intact or -- reacted ) and abnormal , were frequently seen in the cumulus mass , free in the intercellular spaces or close to the cumulus cells , that can induce sperm capacitation and acrosome reaction .
	manualset3
139339	2	407386	5	NULL	NULL	NULL	NULL	cumulus mass 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Spermatozoa , both normal ( acrosome-intact or -- reacted ) and abnormal , were frequently seen in the cumulus mass , free in the intercellular spaces or close to the cumulus cells , that can induce sperm capacitation and acrosome reaction .
	manualset3
139340	3	407386	5	NULL	NULL	0	NULL	intercellular spaces	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Spermatozoa , both normal ( acrosome-intact or -- reacted ) and abnormal , were frequently seen in the cumulus mass , free in the intercellular spaces or close to the cumulus cells , that can induce sperm capacitation and acrosome reaction .
	manualset3
139341	4	407386	5	NULL	NULL	0	NULL	cumulus cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Spermatozoa , both normal ( acrosome-intact or -- reacted ) and abnormal , were frequently seen in the cumulus mass , free in the intercellular spaces or close to the cumulus cells , that can induce sperm capacitation and acrosome reaction .
	manualset3
139342	5	407386	5	NULL	NULL	0	NULL	sperm capacitation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Spermatozoa , both normal ( acrosome-intact or -- reacted ) and abnormal , were frequently seen in the cumulus mass , free in the intercellular spaces or close to the cumulus cells , that can induce sperm capacitation and acrosome reaction .
	manualset3
139343	6	407386	5	NULL	NULL	0	NULL	acrosome reaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Spermatozoa , both normal ( acrosome-intact or -- reacted ) and abnormal , were frequently seen in the cumulus mass , free in the intercellular spaces or close to the cumulus cells , that can induce sperm capacitation and acrosome reaction .
	manualset3
139344	1	407387	5	NULL	NULL	0	NULL	Spermatozoa 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Spermatozoa incubated with 3 x 106 PMN ml-1 revealed a significant ( P = 0.003 ) decrease in progressive motility after 2 h. This decrease remained weakly significant ( P = 0.024 ) after 4 and 6 h. Lymphocytes and monocytes had no effect on sperm motility .
	manualset3
139345	2	407387	5	NULL	NULL	0	NULL	3 x 106 PMN ml-1 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Spermatozoa incubated with 3 x 106 PMN ml-1 revealed a significant ( P = 0.003 ) decrease in progressive motility after 2 h. This decrease remained weakly significant ( P = 0.024 ) after 4 and 6 h. Lymphocytes and monocytes had no effect on sperm motility .
	manualset3
139346	3	407387	5	NULL	NULL	0	NULL	 P = 0.003 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Spermatozoa incubated with 3 x 106 PMN ml-1 revealed a significant ( P = 0.003 ) decrease in progressive motility after 2 h. This decrease remained weakly significant ( P = 0.024 ) after 4 and 6 h. Lymphocytes and monocytes had no effect on sperm motility .
	manualset3
139347	4	407387	5	NULL	NULL	NULL	NULL	progressive motility	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Spermatozoa incubated with 3 x 106 PMN ml-1 revealed a significant ( P = 0.003 ) decrease in progressive motility after 2 h. This decrease remained weakly significant ( P = 0.024 ) after 4 and 6 h. Lymphocytes and monocytes had no effect on sperm motility .
	manualset3
139348	5	407387	5	NULL	NULL	0	NULL	2 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Spermatozoa incubated with 3 x 106 PMN ml-1 revealed a significant ( P = 0.003 ) decrease in progressive motility after 2 h. This decrease remained weakly significant ( P = 0.024 ) after 4 and 6 h. Lymphocytes and monocytes had no effect on sperm motility .
	manualset3
139349	6	407387	5	NULL	NULL	0	NULL	P = 0.024	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Spermatozoa incubated with 3 x 106 PMN ml-1 revealed a significant ( P = 0.003 ) decrease in progressive motility after 2 h. This decrease remained weakly significant ( P = 0.024 ) after 4 and 6 h. Lymphocytes and monocytes had no effect on sperm motility .
	manualset3
139350	7	407387	5	NULL	NULL	0	NULL	4 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Spermatozoa incubated with 3 x 106 PMN ml-1 revealed a significant ( P = 0.003 ) decrease in progressive motility after 2 h. This decrease remained weakly significant ( P = 0.024 ) after 4 and 6 h. Lymphocytes and monocytes had no effect on sperm motility .
	manualset3
139351	8	407387	5	NULL	NULL	0	NULL	6 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Spermatozoa incubated with 3 x 106 PMN ml-1 revealed a significant ( P = 0.003 ) decrease in progressive motility after 2 h. This decrease remained weakly significant ( P = 0.024 ) after 4 and 6 h. Lymphocytes and monocytes had no effect on sperm motility .
	manualset3
139352	9	407387	5	NULL	NULL	0	NULL	Lymphocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Spermatozoa incubated with 3 x 106 PMN ml-1 revealed a significant ( P = 0.003 ) decrease in progressive motility after 2 h. This decrease remained weakly significant ( P = 0.024 ) after 4 and 6 h. Lymphocytes and monocytes had no effect on sperm motility .
	manualset3
139353	10	407387	5	NULL	NULL	0	NULL	monocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Spermatozoa incubated with 3 x 106 PMN ml-1 revealed a significant ( P = 0.003 ) decrease in progressive motility after 2 h. This decrease remained weakly significant ( P = 0.024 ) after 4 and 6 h. Lymphocytes and monocytes had no effect on sperm motility .
	manualset3
139354	11	407387	5	NULL	NULL	0	NULL	sperm motility	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Spermatozoa incubated with 3 x 106 PMN ml-1 revealed a significant ( P = 0.003 ) decrease in progressive motility after 2 h. This decrease remained weakly significant ( P = 0.024 ) after 4 and 6 h. Lymphocytes and monocytes had no effect on sperm motility .
	manualset3
139691	12	407387	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Spermatozoa incubated with 3 x 106 PMN ml-1 revealed a significant ( P = 0.003 ) decrease in progressive motility after 2 h. This decrease remained weakly significant ( P = 0.024 ) after 4 and 6 h. Lymphocytes and monocytes had no effect on sperm motility .
	manualset3
139355	1	407388	5	NULL	NULL	0	NULL	Spermine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Spermine binding to GC-rich DNA : experimental and theoretical studies .
	manualset3
139356	2	407388	5	NULL	NULL	0	NULL	GC-rich DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Spermine binding to GC-rich DNA : experimental and theoretical studies .
	manualset3
139357	3	407388	5	NULL	NULL	0	NULL	experimental studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spermine binding to GC-rich DNA : experimental and theoretical studies .
	manualset3
139358	4	407388	5	NULL	NULL	0	NULL	theoretical studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spermine binding to GC-rich DNA : experimental and theoretical studies .
	manualset3
139359	1	407389	5	NULL	NULL	0	NULL	Spina bifida occulta	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Spina bifida occulta was revealed postoperatively by X-ray .
	manualset3
139360	2	407389	5	NULL	NULL	NULL	NULL	X-ray	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Spina bifida occulta was revealed postoperatively by X-ray .
	manualset3
139361	1	407390	5	NULL	NULL	0	NULL	Cerebral swelling	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cerebral swelling and edema in the course of internal diseases ) .
	manualset3
139362	2	407390	5	NULL	NULL	0	NULL	edema 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cerebral swelling and edema in the course of internal diseases ) .
	manualset3
139363	3	407390	5	NULL	NULL	0	NULL	internal diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cerebral swelling and edema in the course of internal diseases ) .
	manualset3
139364	1	407391	5	NULL	NULL	0	NULL	peripheral leukocyte migration inhibition test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A peripheral leukocyte migration inhibition test has been used to demonstrate cellular immunity to a protein component of Neisseria gonorrhoeae .
	manualset3
139365	2	407391	5	NULL	NULL	0	NULL	cellular immunity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A peripheral leukocyte migration inhibition test has been used to demonstrate cellular immunity to a protein component of Neisseria gonorrhoeae .
	manualset3
139366	3	407391	5	NULL	NULL	0	NULL	protein component	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A peripheral leukocyte migration inhibition test has been used to demonstrate cellular immunity to a protein component of Neisseria gonorrhoeae .
	manualset3
139367	4	407391	5	NULL	NULL	0	NULL	Neisseria gonorrhoeae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A peripheral leukocyte migration inhibition test has been used to demonstrate cellular immunity to a protein component of Neisseria gonorrhoeae .
	manualset3
139368	1	407392	5	NULL	NULL	0	NULL	Spinal cord tissue levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spinal cord tissue levels of CGRP and IGF-I were increased after the induction of SCI , peaking at 2 h postinduction .
	manualset3
139369	2	407392	5	NULL	NULL	0	NULL	CGRP 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Spinal cord tissue levels of CGRP and IGF-I were increased after the induction of SCI , peaking at 2 h postinduction .
	manualset3
139370	3	407392	5	NULL	NULL	0	NULL	IGF-I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Spinal cord tissue levels of CGRP and IGF-I were increased after the induction of SCI , peaking at 2 h postinduction .
	manualset3
139371	4	407392	5	NULL	NULL	0	NULL	induction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Spinal cord tissue levels of CGRP and IGF-I were increased after the induction of SCI , peaking at 2 h postinduction .
	manualset3
139372	5	407392	5	NULL	NULL	0	NULL	SCI 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Spinal cord tissue levels of CGRP and IGF-I were increased after the induction of SCI , peaking at 2 h postinduction .
	manualset3
139373	6	407392	5	NULL	NULL	0	NULL	2 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Spinal cord tissue levels of CGRP and IGF-I were increased after the induction of SCI , peaking at 2 h postinduction .
	manualset3
139374	7	407392	5	NULL	NULL	0	NULL	postinduction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Spinal cord tissue levels of CGRP and IGF-I were increased after the induction of SCI , peaking at 2 h postinduction .
	manualset3
139375	1	407393	5	NULL	NULL	0	NULL	Spinal fusion surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Spinal fusion surgery generally involves the insertion of screws in the pedicle , a three-dimensional ( 3-D ) process that requires great skill if serious consequences are to be avoided .
	manualset3
139376	2	407393	5	NULL	NULL	0	NULL	insertion 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Spinal fusion surgery generally involves the insertion of screws in the pedicle , a three-dimensional ( 3-D ) process that requires great skill if serious consequences are to be avoided .
	manualset3
139377	3	407393	5	NULL	NULL	0	NULL	screws 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Spinal fusion surgery generally involves the insertion of screws in the pedicle , a three-dimensional ( 3-D ) process that requires great skill if serious consequences are to be avoided .
	manualset3
139378	4	407393	5	NULL	NULL	0	NULL	pedicle 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Spinal fusion surgery generally involves the insertion of screws in the pedicle , a three-dimensional ( 3-D ) process that requires great skill if serious consequences are to be avoided .
	manualset3
139379	5	407393	5	NULL	NULL	0	NULL	three-dimensional ( 3-D ) process	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Spinal fusion surgery generally involves the insertion of screws in the pedicle , a three-dimensional ( 3-D ) process that requires great skill if serious consequences are to be avoided .
	manualset3
139380	6	407393	5	NULL	NULL	0	NULL	skill 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Spinal fusion surgery generally involves the insertion of screws in the pedicle , a three-dimensional ( 3-D ) process that requires great skill if serious consequences are to be avoided .
	manualset3
139381	7	407393	5	NULL	NULL	0	NULL	serious consequences	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Spinal fusion surgery generally involves the insertion of screws in the pedicle , a three-dimensional ( 3-D ) process that requires great skill if serious consequences are to be avoided .
	manualset3
139382	1	407394	5	NULL	NULL	0	NULL	Spinal ganglion cytological responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Spinal ganglion cytological responses to axon and to dendrite sectioning .
	manualset3
139383	2	407394	5	NULL	NULL	0	NULL	axon sectioning 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Spinal ganglion cytological responses to axon and to dendrite sectioning .
	manualset3
139384	3	407394	5	NULL	NULL	0	NULL	dendrite sectioning 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Spinal ganglion cytological responses to axon and to dendrite sectioning .
	manualset3
139385	1	407395	5	NULL	NULL	0	NULL	Spirometric indices	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spirometric indices , 6 min walking distance , symptom scores and extra beta-agonist use were no different between MDI and NEB treatment fortnights in the outpatient study .
	manualset3
139386	2	407395	5	NULL	NULL	0	NULL	6 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Spirometric indices , 6 min walking distance , symptom scores and extra beta-agonist use were no different between MDI and NEB treatment fortnights in the outpatient study .
	manualset3
139387	3	407395	5	NULL	NULL	0	NULL	walking distance	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spirometric indices , 6 min walking distance , symptom scores and extra beta-agonist use were no different between MDI and NEB treatment fortnights in the outpatient study .
	manualset3
139388	4	407395	5	NULL	NULL	0	NULL	symptom scores	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spirometric indices , 6 min walking distance , symptom scores and extra beta-agonist use were no different between MDI and NEB treatment fortnights in the outpatient study .
	manualset3
139389	5	407395	5	NULL	NULL	0	NULL	beta-agonist	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Spirometric indices , 6 min walking distance , symptom scores and extra beta-agonist use were no different between MDI and NEB treatment fortnights in the outpatient study .
	manualset3
139390	6	407395	5	NULL	NULL	0	NULL	MDI treatment fortnights	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Spirometric indices , 6 min walking distance , symptom scores and extra beta-agonist use were no different between MDI and NEB treatment fortnights in the outpatient study .
	manualset3
139391	7	407395	5	NULL	NULL	0	NULL	NEB treatment fortnights	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Spirometric indices , 6 min walking distance , symptom scores and extra beta-agonist use were no different between MDI and NEB treatment fortnights in the outpatient study .
	manualset3
139392	8	407395	5	NULL	NULL	0	NULL	outpatient study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spirometric indices , 6 min walking distance , symptom scores and extra beta-agonist use were no different between MDI and NEB treatment fortnights in the outpatient study .
	manualset3
139393	1	407396	5	NULL	NULL	0	NULL	Spleen DCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Spleen DCs were cultured with HBsAg ( 100 microg ) for 24 h to produce HBsAg-pulsed DCs .
	manualset3
139394	2	407396	5	NULL	NULL	0	NULL	HBsAg 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Spleen DCs were cultured with HBsAg ( 100 microg ) for 24 h to produce HBsAg-pulsed DCs .
	manualset3
139395	3	407396	5	NULL	NULL	0	NULL	100 microg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Spleen DCs were cultured with HBsAg ( 100 microg ) for 24 h to produce HBsAg-pulsed DCs .
	manualset3
139396	4	407396	5	NULL	NULL	0	NULL	24 h 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Spleen DCs were cultured with HBsAg ( 100 microg ) for 24 h to produce HBsAg-pulsed DCs .
	manualset3
139397	5	407396	5	NULL	NULL	0	NULL	HBsAg-pulsed DCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Spleen DCs were cultured with HBsAg ( 100 microg ) for 24 h to produce HBsAg-pulsed DCs .
	manualset3
139398	1	407397	5	NULL	NULL	0	NULL	Spleen cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Spleen cells were sorted by FALS and four different populations of NCC detected .
	manualset3
139399	2	407397	5	NULL	NULL	0	NULL	FALS 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spleen cells were sorted by FALS and four different populations of NCC detected .
	manualset3
139400	3	407397	5	NULL	NULL	0	NULL	populations 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Spleen cells were sorted by FALS and four different populations of NCC detected .
	manualset3
139401	4	407397	5	NULL	NULL	0	NULL	NCC 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Spleen cells were sorted by FALS and four different populations of NCC detected .
	manualset3
139402	1	407398	5	NULL	NULL	0	NULL	Splenectomy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Splenectomy generally reduced the cytotoxic activity and virus titers of lymphocytes from both groups , and thymosin administration further reduced the cytotoxic response .
	manualset3
139403	2	407398	5	NULL	NULL	0	NULL	cytotoxic activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Splenectomy generally reduced the cytotoxic activity and virus titers of lymphocytes from both groups , and thymosin administration further reduced the cytotoxic response .
	manualset3
139404	3	407398	5	NULL	NULL	0	NULL	virus titers	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Splenectomy generally reduced the cytotoxic activity and virus titers of lymphocytes from both groups , and thymosin administration further reduced the cytotoxic response .
	manualset3
139405	4	407398	5	NULL	NULL	0	NULL	lymphocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Splenectomy generally reduced the cytotoxic activity and virus titers of lymphocytes from both groups , and thymosin administration further reduced the cytotoxic response .
	manualset3
139406	5	407398	5	NULL	NULL	0	NULL	groups 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Splenectomy generally reduced the cytotoxic activity and virus titers of lymphocytes from both groups , and thymosin administration further reduced the cytotoxic response .
	manualset3
139407	6	407398	5	NULL	NULL	0	NULL	thymosin administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Splenectomy generally reduced the cytotoxic activity and virus titers of lymphocytes from both groups , and thymosin administration further reduced the cytotoxic response .
	manualset3
139408	7	407398	5	NULL	NULL	0	NULL	cytotoxic response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Splenectomy generally reduced the cytotoxic activity and virus titers of lymphocytes from both groups , and thymosin administration further reduced the cytotoxic response .
	manualset3
139409	1	407399	5	NULL	NULL	0	NULL	Splenic gonadal fusion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Splenic gonadal fusion with persistent mllerian duct syndrome .
	manualset3
139410	2	407399	5	NULL	NULL	0	NULL	mllerian duct syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Splenic gonadal fusion with persistent mllerian duct syndrome .
	manualset3
139411	1	407400	5	NULL	NULL	0	NULL	Split-dose radiotherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Split-dose radiotherapy for radioresistant bone and soft tissue sarcoma : ten years ' experience .
	manualset3
139412	2	407400	5	NULL	NULL	NULL	NULL	radioresistant bone sarcoma 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Split-dose radiotherapy for radioresistant bone and soft tissue sarcoma : ten years ' experience .
	manualset3
139413	3	407400	5	NULL	NULL	0	NULL	 soft tissue sarcoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Split-dose radiotherapy for radioresistant bone and soft tissue sarcoma : ten years ' experience .
	manualset3
139414	4	407400	5	NULL	NULL	0	NULL	 ten years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Split-dose radiotherapy for radioresistant bone and soft tissue sarcoma : ten years ' experience .
	manualset3
139415	5	407400	5	NULL	NULL	0	NULL	experience 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Split-dose radiotherapy for radioresistant bone and soft tissue sarcoma : ten years ' experience .
	manualset3
139416	1	407401	5	NULL	NULL	0	NULL	Split-skin graft	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Split-skin graft in the management of diabetic foot ulcers .
	manualset3
139417	2	407401	5	NULL	NULL	0	NULL	management 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Split-skin graft in the management of diabetic foot ulcers .
	manualset3
139418	3	407401	5	NULL	NULL	0	NULL	diabetic foot ulcers	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Split-skin graft in the management of diabetic foot ulcers .
	manualset3
139419	1	407402	5	NULL	NULL	0	NULL	Spondylitic heart disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Spondylitic heart disease : a case report .
	manualset3
139420	2	407402	5	NULL	NULL	0	NULL	case report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Spondylitic heart disease : a case report .
	manualset3
139421	1	407403	5	NULL	NULL	NULL	NULL	Spontaneous closure	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Spontaneous closure of interatrial septal openings in infants : an echocardiographic study .
	manualset3
139422	2	407403	5	NULL	NULL	0	NULL	interatrial septal openings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous closure of interatrial septal openings in infants : an echocardiographic study .
	manualset3
139423	3	407403	5	NULL	NULL	0	NULL	infants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous closure of interatrial septal openings in infants : an echocardiographic study .
	manualset3
139424	4	407403	5	NULL	NULL	0	NULL	echocardiographic study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous closure of interatrial septal openings in infants : an echocardiographic study .
	manualset3
139425	1	407404	5	NULL	NULL	0	NULL	Spontaneous coronary artery dissection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous coronary artery dissection : aggressive vs. conservative therapy .
	manualset3
139426	2	407404	5	NULL	NULL	0	NULL	aggressive therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous coronary artery dissection : aggressive vs. conservative therapy .
	manualset3
139427	3	407404	5	NULL	NULL	0	NULL	conservative therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous coronary artery dissection : aggressive vs. conservative therapy .
	manualset3
139428	1	407405	5	NULL	NULL	0	NULL	Spontaneous discharge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous discharge was increased in the five cells in which it was present ( P & lt ; 0.05 ) .
	manualset3
139429	2	407405	5	NULL	NULL	0	NULL	five 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous discharge was increased in the five cells in which it was present ( P & lt ; 0.05 ) .
	manualset3
139430	3	407405	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous discharge was increased in the five cells in which it was present ( P & lt ; 0.05 ) .
	manualset3
139431	4	407405	5	NULL	NULL	0	NULL	 P & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous discharge was increased in the five cells in which it was present ( P & lt ; 0.05 ) .
	manualset3
139432	1	407406	5	NULL	NULL	0	NULL	pertussis toxin-sensitive G protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A pertussis toxin-sensitive G protein in hippocampal long-term potentiation .
	manualset3
139433	2	407406	5	NULL	NULL	0	NULL	hippocampal long-term potentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A pertussis toxin-sensitive G protein in hippocampal long-term potentiation .
	manualset3
139434	1	407407	5	NULL	NULL	0	NULL	Spontaneous reduction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous reduction of leukemic lymphoma cells possibly by anti-tumor antibody-mediated phagocytosis ; a kappa lambda-dual-positive B cell lymphoma .
	manualset3
139435	2	407407	5	NULL	NULL	0	NULL	leukemic lymphoma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous reduction of leukemic lymphoma cells possibly by anti-tumor antibody-mediated phagocytosis ; a kappa lambda-dual-positive B cell lymphoma .
	manualset3
139436	3	407407	5	NULL	NULL	0	NULL	anti-tumor antibody-mediated phagocytosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous reduction of leukemic lymphoma cells possibly by anti-tumor antibody-mediated phagocytosis ; a kappa lambda-dual-positive B cell lymphoma .
	manualset3
139437	4	407407	5	NULL	NULL	0	NULL	kappa lambda-dual-positive B cell lymphoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous reduction of leukemic lymphoma cells possibly by anti-tumor antibody-mediated phagocytosis ; a kappa lambda-dual-positive B cell lymphoma .
	manualset3
139438	1	407408	5	NULL	NULL	0	NULL	Spontaneous reduction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous reduction of mixed 2 , 2 ' - bipyridine/methylamine/chloro complexes of Pt ( IV ) in water in the presence of light is accompanied by complex isomerization , loss of methylamine , and formation of a strong oxidant , presumably HOCl .
	manualset3
139439	2	407408	5	NULL	NULL	0	NULL	2 , 2 ' - bipyridine/methylamine/chloro complexes of Pt ( IV )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous reduction of mixed 2 , 2 ' - bipyridine/methylamine/chloro complexes of Pt ( IV ) in water in the presence of light is accompanied by complex isomerization , loss of methylamine , and formation of a strong oxidant , presumably HOCl .
	manualset3
139440	3	407408	5	NULL	NULL	0	NULL	water 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous reduction of mixed 2 , 2 ' - bipyridine/methylamine/chloro complexes of Pt ( IV ) in water in the presence of light is accompanied by complex isomerization , loss of methylamine , and formation of a strong oxidant , presumably HOCl .
	manualset3
139441	4	407408	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous reduction of mixed 2 , 2 ' - bipyridine/methylamine/chloro complexes of Pt ( IV ) in water in the presence of light is accompanied by complex isomerization , loss of methylamine , and formation of a strong oxidant , presumably HOCl .
	manualset3
139442	5	407408	5	NULL	NULL	0	NULL	light 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous reduction of mixed 2 , 2 ' - bipyridine/methylamine/chloro complexes of Pt ( IV ) in water in the presence of light is accompanied by complex isomerization , loss of methylamine , and formation of a strong oxidant , presumably HOCl .
	manualset3
139443	6	407408	5	NULL	NULL	0	NULL	complex isomerization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous reduction of mixed 2 , 2 ' - bipyridine/methylamine/chloro complexes of Pt ( IV ) in water in the presence of light is accompanied by complex isomerization , loss of methylamine , and formation of a strong oxidant , presumably HOCl .
	manualset3
139444	7	407408	5	NULL	NULL	0	NULL	loss 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous reduction of mixed 2 , 2 ' - bipyridine/methylamine/chloro complexes of Pt ( IV ) in water in the presence of light is accompanied by complex isomerization , loss of methylamine , and formation of a strong oxidant , presumably HOCl .
	manualset3
139445	8	407408	5	NULL	NULL	0	NULL	methylamine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous reduction of mixed 2 , 2 ' - bipyridine/methylamine/chloro complexes of Pt ( IV ) in water in the presence of light is accompanied by complex isomerization , loss of methylamine , and formation of a strong oxidant , presumably HOCl .
	manualset3
139446	9	407408	5	NULL	NULL	0	NULL	formation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous reduction of mixed 2 , 2 ' - bipyridine/methylamine/chloro complexes of Pt ( IV ) in water in the presence of light is accompanied by complex isomerization , loss of methylamine , and formation of a strong oxidant , presumably HOCl .
	manualset3
139447	10	407408	5	NULL	NULL	0	NULL	strong oxidant	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous reduction of mixed 2 , 2 ' - bipyridine/methylamine/chloro complexes of Pt ( IV ) in water in the presence of light is accompanied by complex isomerization , loss of methylamine , and formation of a strong oxidant , presumably HOCl .
	manualset3
139448	11	407408	5	NULL	NULL	0	NULL	HOCl 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous reduction of mixed 2 , 2 ' - bipyridine/methylamine/chloro complexes of Pt ( IV ) in water in the presence of light is accompanied by complex isomerization , loss of methylamine , and formation of a strong oxidant , presumably HOCl .
	manualset3
139449	1	407409	5	NULL	NULL	0	NULL	Spontaneous regression 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous regression of primary breast lymphoma .
	manualset3
139450	2	407409	5	NULL	NULL	0	NULL	primary breast lymphoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous regression of primary breast lymphoma .
	manualset3
139451	1	407410	5	NULL	NULL	0	NULL	Spontaneous remission	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous remission occurred 9 months to 5 years after diagnosis as evidenced by restoration of normal adrenal function occurring symptomatically in two patients and advent to hypoadrenalism with addisonian crisis in the two others .
	manualset3
139452	2	407410	5	NULL	NULL	0	NULL	 9 months to 5 years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous remission occurred 9 months to 5 years after diagnosis as evidenced by restoration of normal adrenal function occurring symptomatically in two patients and advent to hypoadrenalism with addisonian crisis in the two others .
	manualset3
139453	3	407410	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous remission occurred 9 months to 5 years after diagnosis as evidenced by restoration of normal adrenal function occurring symptomatically in two patients and advent to hypoadrenalism with addisonian crisis in the two others .
	manualset3
139454	4	407410	5	NULL	NULL	0	NULL	restoration 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous remission occurred 9 months to 5 years after diagnosis as evidenced by restoration of normal adrenal function occurring symptomatically in two patients and advent to hypoadrenalism with addisonian crisis in the two others .
	manualset3
139455	5	407410	5	NULL	NULL	0	NULL	normal adrenal function 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous remission occurred 9 months to 5 years after diagnosis as evidenced by restoration of normal adrenal function occurring symptomatically in two patients and advent to hypoadrenalism with addisonian crisis in the two others .
	manualset3
139456	6	407410	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous remission occurred 9 months to 5 years after diagnosis as evidenced by restoration of normal adrenal function occurring symptomatically in two patients and advent to hypoadrenalism with addisonian crisis in the two others .
	manualset3
139457	7	407410	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous remission occurred 9 months to 5 years after diagnosis as evidenced by restoration of normal adrenal function occurring symptomatically in two patients and advent to hypoadrenalism with addisonian crisis in the two others .
	manualset3
139458	8	407410	5	NULL	NULL	0	NULL	hypoadrenalism 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous remission occurred 9 months to 5 years after diagnosis as evidenced by restoration of normal adrenal function occurring symptomatically in two patients and advent to hypoadrenalism with addisonian crisis in the two others .
	manualset3
139459	9	407410	5	NULL	NULL	0	NULL	addisonian crisis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous remission occurred 9 months to 5 years after diagnosis as evidenced by restoration of normal adrenal function occurring symptomatically in two patients and advent to hypoadrenalism with addisonian crisis in the two others .
	manualset3
139460	10	407410	5	NULL	NULL	0	NULL	two	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous remission occurred 9 months to 5 years after diagnosis as evidenced by restoration of normal adrenal function occurring symptomatically in two patients and advent to hypoadrenalism with addisonian crisis in the two others .
	manualset3
139461	1	407411	5	NULL	NULL	0	NULL	breast microcalcifications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous resolving breast microcalcifications associated with breast carcinoma .
	manualset3
139462	2	407411	5	NULL	NULL	0	NULL	breast carcinoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Spontaneous resolving breast microcalcifications associated with breast carcinoma .
	manualset3
139463	1	407412	5	NULL	NULL	0	NULL	Sporophore production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sporophore production of Agaricus bisporus in aseptic environments .
	manualset3
139464	2	407412	5	NULL	NULL	0	NULL	Agaricus bisporus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sporophore production of Agaricus bisporus in aseptic environments .
	manualset3
139465	3	407412	5	NULL	NULL	0	NULL	aseptic environments	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Sporophore production of Agaricus bisporus in aseptic environments .
	manualset3
139466	1	407413	5	NULL	NULL	0	NULL	pharmacoeconomic review 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A pharmacoeconomic review of its use in the management of asthma .
	manualset3
139467	2	407413	5	NULL	NULL	0	NULL	management 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A pharmacoeconomic review of its use in the management of asthma .
	manualset3
139468	3	407413	5	NULL	NULL	0	NULL	asthma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A pharmacoeconomic review of its use in the management of asthma .
	manualset3
139469	1	407414	5	NULL	NULL	0	NULL	Sporting events 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sporting events affect cardiovascular health through neuroendocrine responses and possibly an increase in high-risk behaviors .
	manualset3
139470	2	407414	5	NULL	NULL	NULL	NULL	cardiovascular health	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Sporting events affect cardiovascular health through neuroendocrine responses and possibly an increase in high-risk behaviors .
	manualset3
139471	3	407414	5	NULL	NULL	0	NULL	neuroendocrine responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sporting events affect cardiovascular health through neuroendocrine responses and possibly an increase in high-risk behaviors .
	manualset3
139472	4	407414	5	NULL	NULL	0	NULL	high-risk behaviors	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sporting events affect cardiovascular health through neuroendocrine responses and possibly an increase in high-risk behaviors .
	manualset3
139473	1	407415	5	NULL	NULL	0	NULL	Sports 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sports related concussion - management in general practice .
	manualset3
139474	2	407415	5	NULL	NULL	0	NULL	concussion - management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Sports related concussion - management in general practice .
	manualset3
139475	3	407415	5	NULL	NULL	0	NULL	general practice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Sports related concussion - management in general practice .
	manualset3
139476	1	407416	5	NULL	NULL	0	NULL	Sprague-Dawley rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sprague-Dawley rats are sensitive to the teratogenic action of AY 9944 , an inhibitor of cholesterol synthesis , but the dose of inhibitor necessary to induce the same rate of characteristic malformations is twice as large for Sprague-Dawley as for Wistar rats .
	manualset3
139477	2	407416	5	NULL	NULL	0	NULL	teratogenic action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sprague-Dawley rats are sensitive to the teratogenic action of AY 9944 , an inhibitor of cholesterol synthesis , but the dose of inhibitor necessary to induce the same rate of characteristic malformations is twice as large for Sprague-Dawley as for Wistar rats .
	manualset3
139478	3	407416	5	NULL	NULL	NULL	NULL	AY 9944 , an inhibitor of cholesterol synthesis	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Sprague-Dawley rats are sensitive to the teratogenic action of AY 9944 , an inhibitor of cholesterol synthesis , but the dose of inhibitor necessary to induce the same rate of characteristic malformations is twice as large for Sprague-Dawley as for Wistar rats .
	manualset3
139479	4	407416	5	NULL	NULL	0	NULL	dose 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sprague-Dawley rats are sensitive to the teratogenic action of AY 9944 , an inhibitor of cholesterol synthesis , but the dose of inhibitor necessary to induce the same rate of characteristic malformations is twice as large for Sprague-Dawley as for Wistar rats .
	manualset3
139480	5	407416	5	NULL	NULL	0	NULL	inhibitor 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Sprague-Dawley rats are sensitive to the teratogenic action of AY 9944 , an inhibitor of cholesterol synthesis , but the dose of inhibitor necessary to induce the same rate of characteristic malformations is twice as large for Sprague-Dawley as for Wistar rats .
	manualset3
139481	6	407416	5	NULL	NULL	0	NULL	rate of characteristic malformations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sprague-Dawley rats are sensitive to the teratogenic action of AY 9944 , an inhibitor of cholesterol synthesis , but the dose of inhibitor necessary to induce the same rate of characteristic malformations is twice as large for Sprague-Dawley as for Wistar rats .
	manualset3
139482	7	407416	5	NULL	NULL	0	NULL	twice 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sprague-Dawley rats are sensitive to the teratogenic action of AY 9944 , an inhibitor of cholesterol synthesis , but the dose of inhibitor necessary to induce the same rate of characteristic malformations is twice as large for Sprague-Dawley as for Wistar rats .
	manualset3
139483	8	407416	5	NULL	NULL	0	NULL	Sprague-Dawley rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sprague-Dawley rats are sensitive to the teratogenic action of AY 9944 , an inhibitor of cholesterol synthesis , but the dose of inhibitor necessary to induce the same rate of characteristic malformations is twice as large for Sprague-Dawley as for Wistar rats .
	manualset3
139484	9	407416	5	NULL	NULL	0	NULL	Wistar rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sprague-Dawley rats are sensitive to the teratogenic action of AY 9944 , an inhibitor of cholesterol synthesis , but the dose of inhibitor necessary to induce the same rate of characteristic malformations is twice as large for Sprague-Dawley as for Wistar rats .
	manualset3
139485	1	407417	5	NULL	NULL	0	NULL	Spruce colonization 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Spruce colonization at treeline : where do those seeds come from ?
	manualset3
139486	2	407417	5	NULL	NULL	0	NULL	treeline 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Spruce colonization at treeline : where do those seeds come from ?
	manualset3
139487	3	407417	5	NULL	NULL	0	NULL	seeds 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Spruce colonization at treeline : where do those seeds come from ?
	manualset3
139488	1	407418	5	NULL	NULL	0	NULL	Squalene 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Squalene , phytene , phytadiene , and pristane were the only terpenoids detected .
	manualset3
139489	2	407418	5	NULL	NULL	0	NULL	phytene 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Squalene , phytene , phytadiene , and pristane were the only terpenoids detected .
	manualset3
139490	3	407418	5	NULL	NULL	0	NULL	phytadiene 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Squalene , phytene , phytadiene , and pristane were the only terpenoids detected .
	manualset3
139491	4	407418	5	NULL	NULL	0	NULL	pristane 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Squalene , phytene , phytadiene , and pristane were the only terpenoids detected .
	manualset3
139492	5	407418	5	NULL	NULL	0	NULL	terpenoids 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Squalene , phytene , phytadiene , and pristane were the only terpenoids detected .
	manualset3
139493	1	407419	5	NULL	NULL	0	NULL	Squamous cell carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Squamous cell carcinoma of the stomach .
	manualset3
139494	2	407419	5	NULL	NULL	0	NULL	stomach 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Squamous cell carcinoma of the stomach .
	manualset3
139495	1	407420	5	NULL	NULL	0	NULL	Src homology 2 domain-containing inositol polyphosphate phosphatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Src homology 2 domain-containing inositol polyphosphate phosphatase regulates NF-kappa B-mediated gene transcription by phagocytic Fc gamma Rs in human myeloid cells .
	manualset3
139496	2	407420	5	NULL	NULL	0	NULL	NF-kappa B-mediated gene transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Src homology 2 domain-containing inositol polyphosphate phosphatase regulates NF-kappa B-mediated gene transcription by phagocytic Fc gamma Rs in human myeloid cells .
	manualset3
139497	3	407420	5	NULL	NULL	0	NULL	Fc gamma Rs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Src homology 2 domain-containing inositol polyphosphate phosphatase regulates NF-kappa B-mediated gene transcription by phagocytic Fc gamma Rs in human myeloid cells .
	manualset3
139498	4	407420	5	NULL	NULL	0	NULL	human myeloid cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Src homology 2 domain-containing inositol polyphosphate phosphatase regulates NF-kappa B-mediated gene transcription by phagocytic Fc gamma Rs in human myeloid cells .
	manualset3
139499	1	407421	5	NULL	NULL	0	NULL	1 , 3 , 5-triazine derivative ( 1 ) , a corticotropin-releasing factor inhibitor 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Stability of the 1 , 3 , 5-triazine derivative ( 1 ) , a corticotropin-releasing factor inhibitor , was studied in acidic solutions and in solid formulations .
	manualset3
139500	2	407421	5	NULL	NULL	0	NULL	acidic solutions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Stability of the 1 , 3 , 5-triazine derivative ( 1 ) , a corticotropin-releasing factor inhibitor , was studied in acidic solutions and in solid formulations .
	manualset3
139501	3	407421	5	NULL	NULL	0	NULL	solid formulations	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Stability of the 1 , 3 , 5-triazine derivative ( 1 ) , a corticotropin-releasing factor inhibitor , was studied in acidic solutions and in solid formulations .
	manualset3
139502	1	407422	5	NULL	NULL	0	NULL	phase II multicenter study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A phase II multicenter study of oxaliplatin in combination with paclitaxel in poor prognosis patients who failed cisplatin-based chemotherapy for germ-cell tumors .
	manualset3
139503	2	407422	5	NULL	NULL	0	NULL	oxaliplatin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A phase II multicenter study of oxaliplatin in combination with paclitaxel in poor prognosis patients who failed cisplatin-based chemotherapy for germ-cell tumors .
	manualset3
139504	3	407422	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A phase II multicenter study of oxaliplatin in combination with paclitaxel in poor prognosis patients who failed cisplatin-based chemotherapy for germ-cell tumors .
	manualset3
139505	4	407422	5	NULL	NULL	0	NULL	paclitaxel 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A phase II multicenter study of oxaliplatin in combination with paclitaxel in poor prognosis patients who failed cisplatin-based chemotherapy for germ-cell tumors .
	manualset3
139506	5	407422	5	NULL	NULL	0	NULL	poor prognosis patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A phase II multicenter study of oxaliplatin in combination with paclitaxel in poor prognosis patients who failed cisplatin-based chemotherapy for germ-cell tumors .
	manualset3
139507	6	407422	5	NULL	NULL	0	NULL	cisplatin-based chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A phase II multicenter study of oxaliplatin in combination with paclitaxel in poor prognosis patients who failed cisplatin-based chemotherapy for germ-cell tumors .
	manualset3
139508	7	407422	5	NULL	NULL	NULL	NULL	germ-cell tumors	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A phase II multicenter study of oxaliplatin in combination with paclitaxel in poor prognosis patients who failed cisplatin-based chemotherapy for germ-cell tumors .
	manualset3
139509	1	407423	5	NULL	NULL	0	NULL	Stabilization 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stabilization of RNA during laser capture microdissection by performing experiments under argon atmosphere or using ethanol as a solvent in staining solutions .
	manualset3
139510	2	407423	5	NULL	NULL	0	NULL	RNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Stabilization of RNA during laser capture microdissection by performing experiments under argon atmosphere or using ethanol as a solvent in staining solutions .
	manualset3
139511	3	407423	5	NULL	NULL	0	NULL	laser capture microdissection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stabilization of RNA during laser capture microdissection by performing experiments under argon atmosphere or using ethanol as a solvent in staining solutions .
	manualset3
139512	4	407423	5	NULL	NULL	0	NULL	experiments 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stabilization of RNA during laser capture microdissection by performing experiments under argon atmosphere or using ethanol as a solvent in staining solutions .
	manualset3
139513	5	407423	5	NULL	NULL	0	NULL	argon atmosphere	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Stabilization of RNA during laser capture microdissection by performing experiments under argon atmosphere or using ethanol as a solvent in staining solutions .
	manualset3
139514	6	407423	5	NULL	NULL	0	NULL	ethanol 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Stabilization of RNA during laser capture microdissection by performing experiments under argon atmosphere or using ethanol as a solvent in staining solutions .
	manualset3
139515	7	407423	5	NULL	NULL	0	NULL	solvent 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Stabilization of RNA during laser capture microdissection by performing experiments under argon atmosphere or using ethanol as a solvent in staining solutions .
	manualset3
139516	8	407423	5	NULL	NULL	0	NULL	staining solutions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Stabilization of RNA during laser capture microdissection by performing experiments under argon atmosphere or using ethanol as a solvent in staining solutions .
	manualset3
139517	1	407424	5	NULL	NULL	0	NULL	Stabilization 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stabilization of wild-type p53 by hypoxia-inducible factor 1alpha .
	manualset3
139518	2	407424	5	NULL	NULL	0	NULL	wild-type p53 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Stabilization of wild-type p53 by hypoxia-inducible factor 1alpha .
	manualset3
139519	3	407424	5	NULL	NULL	0	NULL	 hypoxia-inducible factor 1alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Stabilization of wild-type p53 by hypoxia-inducible factor 1alpha .
	manualset3
139520	1	407425	5	NULL	NULL	0	NULL	activated-clamped state 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stabilizing the activated-clamped state at separations of less than 9 nm requires the accessory helix of CPX , which prevents membrane-proximal assembly of SNAREpins .
	manualset3
139521	2	407425	5	NULL	NULL	0	NULL	separations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Stabilizing the activated-clamped state at separations of less than 9 nm requires the accessory helix of CPX , which prevents membrane-proximal assembly of SNAREpins .
	manualset3
139522	3	407425	5	NULL	NULL	0	NULL	9 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Stabilizing the activated-clamped state at separations of less than 9 nm requires the accessory helix of CPX , which prevents membrane-proximal assembly of SNAREpins .
	manualset3
139523	4	407425	5	NULL	NULL	0	NULL	accessory helix 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Stabilizing the activated-clamped state at separations of less than 9 nm requires the accessory helix of CPX , which prevents membrane-proximal assembly of SNAREpins .
	manualset3
139524	5	407425	5	NULL	NULL	0	NULL	CPX 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Stabilizing the activated-clamped state at separations of less than 9 nm requires the accessory helix of CPX , which prevents membrane-proximal assembly of SNAREpins .
	manualset3
139525	6	407425	5	NULL	NULL	0	NULL	membrane-proximal assembly 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stabilizing the activated-clamped state at separations of less than 9 nm requires the accessory helix of CPX , which prevents membrane-proximal assembly of SNAREpins .
	manualset3
139526	7	407425	5	NULL	NULL	0	NULL	SNAREpins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Stabilizing the activated-clamped state at separations of less than 9 nm requires the accessory helix of CPX , which prevents membrane-proximal assembly of SNAREpins .
	manualset3
139527	1	407426	5	NULL	NULL	0	NULL	Stable iodinated polypeptide hormones	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Stable iodinated polypeptide hormones prepared by polyacrylamide gel electrophoresis .
	manualset3
139528	2	407426	5	NULL	NULL	0	NULL	polyacrylamide gel electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stable iodinated polypeptide hormones prepared by polyacrylamide gel electrophoresis .
	manualset3
139529	1	407427	5	NULL	NULL	0	NULL	psychosocial resources 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stable psychosocial resources ( i.e. , education , being married , and positive coping styles ) were associated with better chronic glycemic control , while stress and regimen nonadherence were associated with worse transient glycemic control .
	manualset3
139530	2	407427	5	NULL	NULL	0	NULL	education 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stable psychosocial resources ( i.e. , education , being married , and positive coping styles ) were associated with better chronic glycemic control , while stress and regimen nonadherence were associated with worse transient glycemic control .
	manualset3
139531	3	407427	5	NULL	NULL	0	NULL	positive coping styles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Stable psychosocial resources ( i.e. , education , being married , and positive coping styles ) were associated with better chronic glycemic control , while stress and regimen nonadherence were associated with worse transient glycemic control .
	manualset3
139532	4	407427	5	NULL	NULL	0	NULL	chronic glycemic control	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Stable psychosocial resources ( i.e. , education , being married , and positive coping styles ) were associated with better chronic glycemic control , while stress and regimen nonadherence were associated with worse transient glycemic control .
	manualset3
139533	5	407427	5	NULL	NULL	0	NULL	stress 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Stable psychosocial resources ( i.e. , education , being married , and positive coping styles ) were associated with better chronic glycemic control , while stress and regimen nonadherence were associated with worse transient glycemic control .
	manualset3
139534	6	407427	5	NULL	NULL	0	NULL	regimen nonadherence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Stable psychosocial resources ( i.e. , education , being married , and positive coping styles ) were associated with better chronic glycemic control , while stress and regimen nonadherence were associated with worse transient glycemic control .
	manualset3
139535	7	407427	5	NULL	NULL	0	NULL	worse transient glycemic control	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Stable psychosocial resources ( i.e. , education , being married , and positive coping styles ) were associated with better chronic glycemic control , while stress and regimen nonadherence were associated with worse transient glycemic control .
	manualset3
139536	1	407428	5	NULL	NULL	0	NULL	transposon-generated auxotrophic mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stable transposon-generated auxotrophic mutations in aroA , purA , and purE or aroA and purA together were introduced into Salmonella typhimurium strains which were virulent in mice .
	manualset3
139537	2	407428	5	NULL	NULL	0	NULL	aroA 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Stable transposon-generated auxotrophic mutations in aroA , purA , and purE or aroA and purA together were introduced into Salmonella typhimurium strains which were virulent in mice .
	manualset3
139538	3	407428	5	NULL	NULL	0	NULL	purA 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Stable transposon-generated auxotrophic mutations in aroA , purA , and purE or aroA and purA together were introduced into Salmonella typhimurium strains which were virulent in mice .
	manualset3
139539	4	407428	5	NULL	NULL	0	NULL	purE 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Stable transposon-generated auxotrophic mutations in aroA , purA , and purE or aroA and purA together were introduced into Salmonella typhimurium strains which were virulent in mice .
	manualset3
139540	5	407428	5	NULL	NULL	0	NULL	aroA 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Stable transposon-generated auxotrophic mutations in aroA , purA , and purE or aroA and purA together were introduced into Salmonella typhimurium strains which were virulent in mice .
	manualset3
139541	6	407428	5	NULL	NULL	0	NULL	purA 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Stable transposon-generated auxotrophic mutations in aroA , purA , and purE or aroA and purA together were introduced into Salmonella typhimurium strains which were virulent in mice .
	manualset3
139542	7	407428	5	NULL	NULL	0	NULL	Salmonella typhimurium strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Stable transposon-generated auxotrophic mutations in aroA , purA , and purE or aroA and purA together were introduced into Salmonella typhimurium strains which were virulent in mice .
	manualset3
139543	8	407428	5	NULL	NULL	0	NULL	mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Stable transposon-generated auxotrophic mutations in aroA , purA , and purE or aroA and purA together were introduced into Salmonella typhimurium strains which were virulent in mice .
	manualset3
139544	1	407429	5	NULL	NULL	0	NULL	Staff management 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Staff management and clinical considerations for treatment of HIV ( AIDS ) virus-infected patients .
	manualset3
139545	2	407429	5	NULL	NULL	0	NULL	clinical considerations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Staff management and clinical considerations for treatment of HIV ( AIDS ) virus-infected patients .
	manualset3
139546	3	407429	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Staff management and clinical considerations for treatment of HIV ( AIDS ) virus-infected patients .
	manualset3
139547	4	407429	5	NULL	NULL	0	NULL	HIV ( AIDS ) virus-infected patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Staff management and clinical considerations for treatment of HIV ( AIDS ) virus-infected patients .
	manualset3
139548	1	407430	5	NULL	NULL	0	NULL	Stage-dependent effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Stage-dependent effect of leptin on development of porcine embryos derived from parthenogenetic activation and transgenic somatic cell nuclear transfer .
	manualset3
139549	2	407430	5	NULL	NULL	0	NULL	leptin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Stage-dependent effect of leptin on development of porcine embryos derived from parthenogenetic activation and transgenic somatic cell nuclear transfer .
	manualset3
139550	3	407430	5	NULL	NULL	0	NULL	development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stage-dependent effect of leptin on development of porcine embryos derived from parthenogenetic activation and transgenic somatic cell nuclear transfer .
	manualset3
139551	4	407430	5	NULL	NULL	0	NULL	porcine embryos	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Stage-dependent effect of leptin on development of porcine embryos derived from parthenogenetic activation and transgenic somatic cell nuclear transfer .
	manualset3
139552	5	407430	5	NULL	NULL	0	NULL	parthenogenetic activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stage-dependent effect of leptin on development of porcine embryos derived from parthenogenetic activation and transgenic somatic cell nuclear transfer .
	manualset3
139553	6	407430	5	NULL	NULL	0	NULL	transgenic somatic cell nuclear transfer	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stage-dependent effect of leptin on development of porcine embryos derived from parthenogenetic activation and transgenic somatic cell nuclear transfer .
	manualset3
139554	1	407431	5	NULL	NULL	0	NULL	phosphorus-containing hybrid porphyrin 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A phosphorus-containing hybrid porphyrin was successfully prepared via the BF3-promoted dehydrative condensation between sigma4-phosphatripyrrane and 2 , 5-bis ( hydroxy ( phenyl ) methyl ) thiophene .
	manualset3
139555	2	407431	5	NULL	NULL	0	NULL	BF3-promoted dehydrative condensation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A phosphorus-containing hybrid porphyrin was successfully prepared via the BF3-promoted dehydrative condensation between sigma4-phosphatripyrrane and 2 , 5-bis ( hydroxy ( phenyl ) methyl ) thiophene .
	manualset3
139556	3	407431	5	NULL	NULL	0	NULL	sigma4-phosphatripyrrane	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A phosphorus-containing hybrid porphyrin was successfully prepared via the BF3-promoted dehydrative condensation between sigma4-phosphatripyrrane and 2 , 5-bis ( hydroxy ( phenyl ) methyl ) thiophene .
	manualset3
139557	4	407431	5	NULL	NULL	0	NULL	2 , 5-bis ( hydroxy ( phenyl ) methyl ) thiophene	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A phosphorus-containing hybrid porphyrin was successfully prepared via the BF3-promoted dehydrative condensation between sigma4-phosphatripyrrane and 2 , 5-bis ( hydroxy ( phenyl ) methyl ) thiophene .
	manualset3
139558	1	407432	5	NULL	NULL	0	NULL	Stage-dependent regulation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stage-dependent regulation of ovarian pituitary adenylate cyclase-activating polypeptide mRNA levels by GnRH in cultured rat granulosa cells .
	manualset3
139559	2	407432	5	NULL	NULL	0	NULL	ovarian pituitary adenylate cyclase-activating polypeptide mRNA levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stage-dependent regulation of ovarian pituitary adenylate cyclase-activating polypeptide mRNA levels by GnRH in cultured rat granulosa cells .
	manualset3
139560	3	407432	5	NULL	NULL	0	NULL	GnRH 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Stage-dependent regulation of ovarian pituitary adenylate cyclase-activating polypeptide mRNA levels by GnRH in cultured rat granulosa cells .
	manualset3
139561	4	407432	5	NULL	NULL	0	NULL	cultured rat granulosa cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Stage-dependent regulation of ovarian pituitary adenylate cyclase-activating polypeptide mRNA levels by GnRH in cultured rat granulosa cells .
	manualset3
139562	1	407433	5	NULL	NULL	0	NULL	Stage I 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Stage I is characterized by subfascial congestion , oedema and corona phlebectatica , stage II by induration and stasis dermatitis , stage III by the occurrence of venous ulcers .
	manualset3
139563	2	407433	5	NULL	NULL	0	NULL	subfascial congestion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Stage I is characterized by subfascial congestion , oedema and corona phlebectatica , stage II by induration and stasis dermatitis , stage III by the occurrence of venous ulcers .
	manualset3
139564	3	407433	5	NULL	NULL	0	NULL	oedema 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Stage I is characterized by subfascial congestion , oedema and corona phlebectatica , stage II by induration and stasis dermatitis , stage III by the occurrence of venous ulcers .
	manualset3
139565	4	407433	5	NULL	NULL	NULL	NULL	corona phlebectatica	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Stage I is characterized by subfascial congestion , oedema and corona phlebectatica , stage II by induration and stasis dermatitis , stage III by the occurrence of venous ulcers .
	manualset3
139566	5	407433	5	NULL	NULL	0	NULL	 stage II	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Stage I is characterized by subfascial congestion , oedema and corona phlebectatica , stage II by induration and stasis dermatitis , stage III by the occurrence of venous ulcers .
	manualset3
139567	6	407433	5	NULL	NULL	0	NULL	induration 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Stage I is characterized by subfascial congestion , oedema and corona phlebectatica , stage II by induration and stasis dermatitis , stage III by the occurrence of venous ulcers .
	manualset3
139568	7	407433	5	NULL	NULL	0	NULL	stasis dermatitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Stage I is characterized by subfascial congestion , oedema and corona phlebectatica , stage II by induration and stasis dermatitis , stage III by the occurrence of venous ulcers .
	manualset3
139569	8	407433	5	NULL	NULL	0	NULL	stage III	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Stage I is characterized by subfascial congestion , oedema and corona phlebectatica , stage II by induration and stasis dermatitis , stage III by the occurrence of venous ulcers .
	manualset3
139570	9	407433	5	NULL	NULL	0	NULL	occurrence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Stage I is characterized by subfascial congestion , oedema and corona phlebectatica , stage II by induration and stasis dermatitis , stage III by the occurrence of venous ulcers .
	manualset3
139571	10	407433	5	NULL	NULL	0	NULL	venous ulcers	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Stage I is characterized by subfascial congestion , oedema and corona phlebectatica , stage II by induration and stasis dermatitis , stage III by the occurrence of venous ulcers .
	manualset3
139572	1	407434	5	NULL	NULL	0	NULL	Staging 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Staging anorexia nervosa could improve outcomes , say experts .
	manualset3
139573	2	407434	5	NULL	NULL	0	NULL	anorexia nervosa	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Staging anorexia nervosa could improve outcomes , say experts .
	manualset3
139574	3	407434	5	NULL	NULL	0	NULL	outcomes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Staging anorexia nervosa could improve outcomes , say experts .
	manualset3
139575	4	407434	5	NULL	NULL	0	NULL	experts 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Staging anorexia nervosa could improve outcomes , say experts .
	manualset3
139576	1	407435	5	NULL	NULL	0	NULL	Stagonospora nodorum blotch ( SNB )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Stagonospora nodorum blotch ( SNB ) caused by Stagonospora nodorum is a severe disease of wheat ( Triticum aestivum ) in many areas of the world .
	manualset3
139577	2	407435	5	NULL	NULL	0	NULL	Stagonospora nodorum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Stagonospora nodorum blotch ( SNB ) caused by Stagonospora nodorum is a severe disease of wheat ( Triticum aestivum ) in many areas of the world .
	manualset3
139578	3	407435	5	NULL	NULL	0	NULL	disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Stagonospora nodorum blotch ( SNB ) caused by Stagonospora nodorum is a severe disease of wheat ( Triticum aestivum ) in many areas of the world .
	manualset3
139579	4	407435	5	NULL	NULL	0	NULL	wheat ( Triticum aestivum )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Stagonospora nodorum blotch ( SNB ) caused by Stagonospora nodorum is a severe disease of wheat ( Triticum aestivum ) in many areas of the world .
	manualset3
139580	5	407435	5	NULL	NULL	0	NULL	areas 	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Stagonospora nodorum blotch ( SNB ) caused by Stagonospora nodorum is a severe disease of wheat ( Triticum aestivum ) in many areas of the world .
	manualset3
139581	6	407435	5	NULL	NULL	0	NULL	world 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Stagonospora nodorum blotch ( SNB ) caused by Stagonospora nodorum is a severe disease of wheat ( Triticum aestivum ) in many areas of the world .
	manualset3
139582	1	407436	5	NULL	NULL	0	NULL	NOS III 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Staining for NOS III of spiral ganglion perikarya showed varying intensity .
	manualset3
139583	2	407436	5	NULL	NULL	0	NULL	spiral ganglion perikarya	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Staining for NOS III of spiral ganglion perikarya showed varying intensity .
	manualset3
139584	3	407436	5	NULL	NULL	0	NULL	intensity 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Staining for NOS III of spiral ganglion perikarya showed varying intensity .
	manualset3
142886	4	407436	5	NULL	NULL	0	NULL	Staining 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Staining for NOS III of spiral ganglion perikarya showed varying intensity .
	manualset3
139585	1	407437	5	NULL	NULL	0	NULL	fibrillar actin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Staining of fibrillar actin with fluorescein-phalloidin revealed a similar organization of the actin cytoskeleton on both substrates .
	manualset3
139586	2	407437	5	NULL	NULL	0	NULL	fluorescein-phalloidin	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Staining of fibrillar actin with fluorescein-phalloidin revealed a similar organization of the actin cytoskeleton on both substrates .
	manualset3
139587	3	407437	5	NULL	NULL	0	NULL	organization 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Staining of fibrillar actin with fluorescein-phalloidin revealed a similar organization of the actin cytoskeleton on both substrates .
	manualset3
139588	4	407437	5	NULL	NULL	0	NULL	actin cytoskeleton	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Staining of fibrillar actin with fluorescein-phalloidin revealed a similar organization of the actin cytoskeleton on both substrates .
	manualset3
139589	5	407437	5	NULL	NULL	0	NULL	substrates 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Staining of fibrillar actin with fluorescein-phalloidin revealed a similar organization of the actin cytoskeleton on both substrates .
	manualset3
142887	6	407437	5	NULL	NULL	0	NULL	Staining 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Staining of fibrillar actin with fluorescein-phalloidin revealed a similar organization of the actin cytoskeleton on both substrates .
	manualset3
139590	1	407438	5	NULL	NULL	NULL	NULL	calcification front	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Staining of the calcification front in human bone using contrasting fluorochromes in vitro .
	manualset3
139591	2	407438	5	NULL	NULL	0	NULL	human bone	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Staining of the calcification front in human bone using contrasting fluorochromes in vitro .
	manualset3
139592	3	407438	5	NULL	NULL	0	NULL	fluorochromes 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Staining of the calcification front in human bone using contrasting fluorochromes in vitro .
	manualset3
142888	4	407438	5	NULL	NULL	0	NULL	Staining 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Staining of the calcification front in human bone using contrasting fluorochromes in vitro .
	manualset3
139593	1	407439	5	NULL	NULL	0	NULL	molybdate anions 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Staining with molybdate anions revealed three prominent densities near the center of the trimer that forms the unit cell , coinciding with the location of the beta-helix that was proposed for the structure of PrP ( Sc ) .
	manualset3
139594	2	407439	5	NULL	NULL	0	NULL	three 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Staining with molybdate anions revealed three prominent densities near the center of the trimer that forms the unit cell , coinciding with the location of the beta-helix that was proposed for the structure of PrP ( Sc ) .
	manualset3
139595	3	407439	5	NULL	NULL	0	NULL	densities 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Staining with molybdate anions revealed three prominent densities near the center of the trimer that forms the unit cell , coinciding with the location of the beta-helix that was proposed for the structure of PrP ( Sc ) .
	manualset3
139596	4	407439	5	NULL	NULL	0	NULL	center 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Staining with molybdate anions revealed three prominent densities near the center of the trimer that forms the unit cell , coinciding with the location of the beta-helix that was proposed for the structure of PrP ( Sc ) .
	manualset3
139597	5	407439	5	NULL	NULL	0	NULL	trimer 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Staining with molybdate anions revealed three prominent densities near the center of the trimer that forms the unit cell , coinciding with the location of the beta-helix that was proposed for the structure of PrP ( Sc ) .
	manualset3
139598	6	407439	5	NULL	NULL	0	NULL	unit cell 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Staining with molybdate anions revealed three prominent densities near the center of the trimer that forms the unit cell , coinciding with the location of the beta-helix that was proposed for the structure of PrP ( Sc ) .
	manualset3
139599	7	407439	5	NULL	NULL	0	NULL	location 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Staining with molybdate anions revealed three prominent densities near the center of the trimer that forms the unit cell , coinciding with the location of the beta-helix that was proposed for the structure of PrP ( Sc ) .
	manualset3
139600	8	407439	5	NULL	NULL	0	NULL	beta-helix	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Staining with molybdate anions revealed three prominent densities near the center of the trimer that forms the unit cell , coinciding with the location of the beta-helix that was proposed for the structure of PrP ( Sc ) .
	manualset3
139601	9	407439	5	NULL	NULL	0	NULL	structure 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Staining with molybdate anions revealed three prominent densities near the center of the trimer that forms the unit cell , coinciding with the location of the beta-helix that was proposed for the structure of PrP ( Sc ) .
	manualset3
139602	10	407439	5	NULL	NULL	0	NULL	 PrP ( Sc )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Staining with molybdate anions revealed three prominent densities near the center of the trimer that forms the unit cell , coinciding with the location of the beta-helix that was proposed for the structure of PrP ( Sc ) .
	manualset3
142889	11	407439	5	NULL	NULL	0	NULL	Staining 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Staining with molybdate anions revealed three prominent densities near the center of the trimer that forms the unit cell , coinciding with the location of the beta-helix that was proposed for the structure of PrP ( Sc ) .
	manualset3
139603	1	407440	5	NULL	NULL	0	NULL	Standard atom probe tomography spatial reconstruction techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Standard atom probe tomography spatial reconstruction techniques have been reasonably successful in reproducing single crystal datasets .
	manualset3
139604	2	407440	5	NULL	NULL	0	NULL	single crystal datasets	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Standard atom probe tomography spatial reconstruction techniques have been reasonably successful in reproducing single crystal datasets .
	manualset3
139605	1	407441	5	NULL	NULL	0	NULL	phylogenetic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A phylogenetic analysis showed that JcDof3 was clustered into the same clade with CYCLING DOF FACTOR ( CDF ) , which interacts with F-box protein to regulate photoperiodic flowering .
	manualset3
139606	2	407441	5	NULL	NULL	0	NULL	JcDof3 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A phylogenetic analysis showed that JcDof3 was clustered into the same clade with CYCLING DOF FACTOR ( CDF ) , which interacts with F-box protein to regulate photoperiodic flowering .
	manualset3
139607	3	407441	5	NULL	NULL	0	NULL	clade 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A phylogenetic analysis showed that JcDof3 was clustered into the same clade with CYCLING DOF FACTOR ( CDF ) , which interacts with F-box protein to regulate photoperiodic flowering .
	manualset3
139608	4	407441	5	NULL	NULL	0	NULL	CYCLING DOF FACTOR ( CDF ) 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A phylogenetic analysis showed that JcDof3 was clustered into the same clade with CYCLING DOF FACTOR ( CDF ) , which interacts with F-box protein to regulate photoperiodic flowering .
	manualset3
139609	5	407441	5	NULL	NULL	0	NULL	F-box protein	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A phylogenetic analysis showed that JcDof3 was clustered into the same clade with CYCLING DOF FACTOR ( CDF ) , which interacts with F-box protein to regulate photoperiodic flowering .
	manualset3
139610	6	407441	5	NULL	NULL	0	NULL	photoperiodic flowering 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A phylogenetic analysis showed that JcDof3 was clustered into the same clade with CYCLING DOF FACTOR ( CDF ) , which interacts with F-box protein to regulate photoperiodic flowering .
	manualset3
139611	1	407442	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Standard treatment in advanced ovarian cancer in 2005 : the state of the art .
	manualset3
139612	2	407442	5	NULL	NULL	0	NULL	ovarian cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Standard treatment in advanced ovarian cancer in 2005 : the state of the art .
	manualset3
139613	3	407442	5	NULL	NULL	0	NULL	2005 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Standard treatment in advanced ovarian cancer in 2005 : the state of the art .
	manualset3
139614	4	407442	5	NULL	NULL	0	NULL	state of the art	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Standard treatment in advanced ovarian cancer in 2005 : the state of the art .
	manualset3
139615	1	407443	5	NULL	NULL	0	NULL	Standard 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Standard for maintaining the competence of neonatal nurse practitioners .
	manualset3
139616	2	407443	5	NULL	NULL	0	NULL	competence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Standard for maintaining the competence of neonatal nurse practitioners .
	manualset3
139617	3	407443	5	NULL	NULL	0	NULL	neonatal nurse practitioners	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Standard for maintaining the competence of neonatal nurse practitioners .
	manualset3
139618	1	407444	5	NULL	NULL	0	NULL	Standardized speckle measurement method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Standardized speckle measurement method matched to human speckle perception in laser projection systems .
	manualset3
139619	2	407444	5	NULL	NULL	0	NULL	human speckle perception 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Standardized speckle measurement method matched to human speckle perception in laser projection systems .
	manualset3
139620	3	407444	5	NULL	NULL	0	NULL	laser projection systems	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Standardized speckle measurement method matched to human speckle perception in laser projection systems .
	manualset3
139621	1	407445	5	NULL	NULL	0	NULL	Staphylococcal-mediated worsening of atopic dermatitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Staphylococcal-mediated worsening of atopic dermatitis : many players involved .
	manualset3
139622	2	407445	5	NULL	NULL	0	NULL	players 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Staphylococcal-mediated worsening of atopic dermatitis : many players involved .
	manualset3
139623	1	407446	5	NULL	NULL	0	NULL	pilot study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A pilot study of the effects of flumazenil on symptoms persisting after benzodiazepine withdrawal .
	manualset3
139624	2	407446	5	NULL	NULL	0	NULL	flumazenil 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A pilot study of the effects of flumazenil on symptoms persisting after benzodiazepine withdrawal .
	manualset3
139625	3	407446	5	NULL	NULL	0	NULL	symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A pilot study of the effects of flumazenil on symptoms persisting after benzodiazepine withdrawal .
	manualset3
139626	4	407446	5	NULL	NULL	0	NULL	benzodiazepine withdrawal 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A pilot study of the effects of flumazenil on symptoms persisting after benzodiazepine withdrawal .
	manualset3
139690	5	407446	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A pilot study of the effects of flumazenil on symptoms persisting after benzodiazepine withdrawal .
	manualset3
139627	1	407447	5	NULL	NULL	0	NULL	Staphylococci 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Staphylococci are increasingly aggressive human pathogens suggesting that active evolution is spreading novel virulence and resistance phenotypes .
	manualset3
139628	2	407447	5	NULL	NULL	0	NULL	human pathogens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Staphylococci are increasingly aggressive human pathogens suggesting that active evolution is spreading novel virulence and resistance phenotypes .
	manualset3
139629	3	407447	5	NULL	NULL	0	NULL	active evolution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Staphylococci are increasingly aggressive human pathogens suggesting that active evolution is spreading novel virulence and resistance phenotypes .
	manualset3
139630	4	407447	5	NULL	NULL	0	NULL	novel virulence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Staphylococci are increasingly aggressive human pathogens suggesting that active evolution is spreading novel virulence and resistance phenotypes .
	manualset3
139631	5	407447	5	NULL	NULL	0	NULL	resistance phenotypes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Staphylococci are increasingly aggressive human pathogens suggesting that active evolution is spreading novel virulence and resistance phenotypes .
	manualset3
139632	1	407448	5	NULL	NULL	0	NULL	Staphylococcus aureus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Staphylococcus aureus tricuspid valve endocarditis in young women after gynaecological events .
	manualset3
139633	2	407448	5	NULL	NULL	0	NULL	tricuspid valve endocarditis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Staphylococcus aureus tricuspid valve endocarditis in young women after gynaecological events .
	manualset3
139634	3	407448	5	NULL	NULL	0	NULL	young women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Staphylococcus aureus tricuspid valve endocarditis in young women after gynaecological events .
	manualset3
139635	4	407448	5	NULL	NULL	0	NULL	gynaecological events	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Staphylococcus aureus tricuspid valve endocarditis in young women after gynaecological events .
	manualset3
139636	1	407449	5	NULL	NULL	0	NULL	Staphylococcus epidermidis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Staphylococcus epidermidis is an opportunistic pathogen associated with foreign body infections and nosocomial sepsis .
	manualset3
139637	2	407449	5	NULL	NULL	0	NULL	opportunistic pathogen	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Staphylococcus epidermidis is an opportunistic pathogen associated with foreign body infections and nosocomial sepsis .
	manualset3
139638	3	407449	5	NULL	NULL	0	NULL	foreign body infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Staphylococcus epidermidis is an opportunistic pathogen associated with foreign body infections and nosocomial sepsis .
	manualset3
139639	4	407449	5	NULL	NULL	0	NULL	nosocomial sepsis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Staphylococcus epidermidis is an opportunistic pathogen associated with foreign body infections and nosocomial sepsis .
	manualset3
139640	1	407450	5	NULL	NULL	0	NULL	Statins 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Statins generally offer the best combination of safety and effectiveness .
	manualset3
139641	2	407450	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Statins generally offer the best combination of safety and effectiveness .
	manualset3
139642	3	407450	5	NULL	NULL	0	NULL	safety 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Statins generally offer the best combination of safety and effectiveness .
	manualset3
139643	4	407450	5	NULL	NULL	0	NULL	effectiveness 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Statins generally offer the best combination of safety and effectiveness .
	manualset3
139644	1	407451	5	NULL	NULL	0	NULL	Statistical significant difference 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistical significant difference between early and metastatic stage of colorectal cancer was confirmed in markers : CEA , CA19-9 , CA242 , TPS , TPA , TK , IGF-1 .
	manualset3
139645	2	407451	5	NULL	NULL	0	NULL	early stage of colorectal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistical significant difference between early and metastatic stage of colorectal cancer was confirmed in markers : CEA , CA19-9 , CA242 , TPS , TPA , TK , IGF-1 .
	manualset3
139646	3	407451	5	NULL	NULL	0	NULL	metastatic stage of colorectal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistical significant difference between early and metastatic stage of colorectal cancer was confirmed in markers : CEA , CA19-9 , CA242 , TPS , TPA , TK , IGF-1 .
	manualset3
139647	4	407451	5	NULL	NULL	0	NULL	markers 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistical significant difference between early and metastatic stage of colorectal cancer was confirmed in markers : CEA , CA19-9 , CA242 , TPS , TPA , TK , IGF-1 .
	manualset3
139648	5	407451	5	NULL	NULL	0	NULL	CEA 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistical significant difference between early and metastatic stage of colorectal cancer was confirmed in markers : CEA , CA19-9 , CA242 , TPS , TPA , TK , IGF-1 .
	manualset3
139649	6	407451	5	NULL	NULL	0	NULL	CA19-9	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistical significant difference between early and metastatic stage of colorectal cancer was confirmed in markers : CEA , CA19-9 , CA242 , TPS , TPA , TK , IGF-1 .
	manualset3
139650	7	407451	5	NULL	NULL	0	NULL	CA242 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistical significant difference between early and metastatic stage of colorectal cancer was confirmed in markers : CEA , CA19-9 , CA242 , TPS , TPA , TK , IGF-1 .
	manualset3
139651	8	407451	5	NULL	NULL	0	NULL	TPS 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistical significant difference between early and metastatic stage of colorectal cancer was confirmed in markers : CEA , CA19-9 , CA242 , TPS , TPA , TK , IGF-1 .
	manualset3
139652	9	407451	5	NULL	NULL	0	NULL	TPA 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistical significant difference between early and metastatic stage of colorectal cancer was confirmed in markers : CEA , CA19-9 , CA242 , TPS , TPA , TK , IGF-1 .
	manualset3
139654	10	407451	5	NULL	NULL	NULL	NULL	TK 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Statistical significant difference between early and metastatic stage of colorectal cancer was confirmed in markers : CEA , CA19-9 , CA242 , TPS , TPA , TK , IGF-1 .
	manualset3
139655	11	407451	5	NULL	NULL	NULL	NULL	IGF-1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Statistical significant difference between early and metastatic stage of colorectal cancer was confirmed in markers : CEA , CA19-9 , CA242 , TPS , TPA , TK , IGF-1 .
	manualset3
139656	1	407452	5	NULL	NULL	0	NULL	pilot study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A pilot study of the thiocarbanilide su-1906 in human pulmonary tuberculosis .
	manualset3
139657	2	407452	5	NULL	NULL	0	NULL	thiocarbanilide su-1906	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A pilot study of the thiocarbanilide su-1906 in human pulmonary tuberculosis .
	manualset3
139658	3	407452	5	NULL	NULL	0	NULL	human pulmonary tuberculosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A pilot study of the thiocarbanilide su-1906 in human pulmonary tuberculosis .
	manualset3
139659	1	407453	5	NULL	NULL	0	NULL	concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistically higher concentrations of T ( p less than 0.05 ) , A ( p less than 0.05 ) and DHEAS ( p less than 0.01 ) were observed in postmenopausal women with RA when compared to controls , whereas no differences were found for all other hormones studied .
	manualset3
139660	2	407453	5	NULL	NULL	0	NULL	T ( p less than 0.05 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistically higher concentrations of T ( p less than 0.05 ) , A ( p less than 0.05 ) and DHEAS ( p less than 0.01 ) were observed in postmenopausal women with RA when compared to controls , whereas no differences were found for all other hormones studied .
	manualset3
139661	3	407453	5	NULL	NULL	0	NULL	A ( p less than 0.05 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistically higher concentrations of T ( p less than 0.05 ) , A ( p less than 0.05 ) and DHEAS ( p less than 0.01 ) were observed in postmenopausal women with RA when compared to controls , whereas no differences were found for all other hormones studied .
	manualset3
139662	4	407453	5	NULL	NULL	0	NULL	DHEAS ( p less than 0.01 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistically higher concentrations of T ( p less than 0.05 ) , A ( p less than 0.05 ) and DHEAS ( p less than 0.01 ) were observed in postmenopausal women with RA when compared to controls , whereas no differences were found for all other hormones studied .
	manualset3
139663	5	407453	5	NULL	NULL	0	NULL	postmenopausal women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistically higher concentrations of T ( p less than 0.05 ) , A ( p less than 0.05 ) and DHEAS ( p less than 0.01 ) were observed in postmenopausal women with RA when compared to controls , whereas no differences were found for all other hormones studied .
	manualset3
139664	6	407453	5	NULL	NULL	0	NULL	RA 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistically higher concentrations of T ( p less than 0.05 ) , A ( p less than 0.05 ) and DHEAS ( p less than 0.01 ) were observed in postmenopausal women with RA when compared to controls , whereas no differences were found for all other hormones studied .
	manualset3
139665	7	407453	5	NULL	NULL	0	NULL	controls 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistically higher concentrations of T ( p less than 0.05 ) , A ( p less than 0.05 ) and DHEAS ( p less than 0.01 ) were observed in postmenopausal women with RA when compared to controls , whereas no differences were found for all other hormones studied .
	manualset3
139666	8	407453	5	NULL	NULL	0	NULL	hormones 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistically higher concentrations of T ( p less than 0.05 ) , A ( p less than 0.05 ) and DHEAS ( p less than 0.01 ) were observed in postmenopausal women with RA when compared to controls , whereas no differences were found for all other hormones studied .
	manualset3
142890	9	407453	5	NULL	NULL	0	NULL	differences 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistically higher concentrations of T ( p less than 0.05 ) , A ( p less than 0.05 ) and DHEAS ( p less than 0.01 ) were observed in postmenopausal women with RA when compared to controls , whereas no differences were found for all other hormones studied .
	manualset3
139667	1	407454	5	NULL	NULL	0	NULL	Status 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Status of this controversial superorder has been evaluated using morphology , paleontology , and mitochondrial plus nuclear DNA sequences .
	manualset3
139668	2	407454	5	NULL	NULL	0	NULL	superorder 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Status of this controversial superorder has been evaluated using morphology , paleontology , and mitochondrial plus nuclear DNA sequences .
	manualset3
139669	3	407454	5	NULL	NULL	0	NULL	morphology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Status of this controversial superorder has been evaluated using morphology , paleontology , and mitochondrial plus nuclear DNA sequences .
	manualset3
139670	4	407454	5	NULL	NULL	0	NULL	paleontology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Status of this controversial superorder has been evaluated using morphology , paleontology , and mitochondrial plus nuclear DNA sequences .
	manualset3
139671	5	407454	5	NULL	NULL	0	NULL	mitochondrial plus nuclear DNA sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Status of this controversial superorder has been evaluated using morphology , paleontology , and mitochondrial plus nuclear DNA sequences .
	manualset3
139672	1	407455	5	NULL	NULL	0	NULL	Status 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Status of bacterial colonization , Toll-like receptor expression and nuclear factor-kappa B activation in normal and diseased human livers .
	manualset3
139673	2	407455	5	NULL	NULL	0	NULL	bacterial colonization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Status of bacterial colonization , Toll-like receptor expression and nuclear factor-kappa B activation in normal and diseased human livers .
	manualset3
139674	3	407455	5	NULL	NULL	0	NULL	Toll-like receptor expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Status of bacterial colonization , Toll-like receptor expression and nuclear factor-kappa B activation in normal and diseased human livers .
	manualset3
139675	4	407455	5	NULL	NULL	0	NULL	nuclear factor-kappa B activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Status of bacterial colonization , Toll-like receptor expression and nuclear factor-kappa B activation in normal and diseased human livers .
	manualset3
139676	5	407455	5	NULL	NULL	0	NULL	normal human livers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Status of bacterial colonization , Toll-like receptor expression and nuclear factor-kappa B activation in normal and diseased human livers .
	manualset3
139677	6	407455	5	NULL	NULL	0	NULL	diseased human livers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Status of bacterial colonization , Toll-like receptor expression and nuclear factor-kappa B activation in normal and diseased human livers .
	manualset3
139678	1	407456	5	NULL	NULL	0	NULL	Status 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Status of basic external human fertilization .
	manualset3
139679	2	407456	5	NULL	NULL	0	NULL	external human fertilization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Status of basic external human fertilization .
	manualset3
139680	1	407457	5	NULL	NULL	0	NULL	Status 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Status of lifecare centers in various regions updated .
	manualset3
139681	2	407457	5	NULL	NULL	0	NULL	lifecare centers	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Status of lifecare centers in various regions updated .
	manualset3
139682	3	407457	5	NULL	NULL	0	NULL	various regions 	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Status of lifecare centers in various regions updated .
	manualset3
139683	1	407458	5	NULL	NULL	0	NULL	Status 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Status epilepticus in the elderly : differential diagnosis and treatment .
	manualset3
139684	2	407458	5	NULL	NULL	0	NULL	epilepticus 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Status epilepticus in the elderly : differential diagnosis and treatment .
	manualset3
139685	3	407458	5	NULL	NULL	0	NULL	elderly 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Status epilepticus in the elderly : differential diagnosis and treatment .
	manualset3
139686	4	407458	5	NULL	NULL	0	NULL	differential diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Status epilepticus in the elderly : differential diagnosis and treatment .
	manualset3
139687	5	407458	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Status epilepticus in the elderly : differential diagnosis and treatment .
	manualset3
139688	1	407459	5	NULL	NULL	0	NULL	Staurosporine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Staurosporine had no frequency-dependent effect on force development , kinetics , calcium transient amplitude , or rate of calcium transient decline .
	manualset3
139689	2	407459	5	NULL	NULL	0	NULL	frequency-dependent effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Staurosporine had no frequency-dependent effect on force development , kinetics , calcium transient amplitude , or rate of calcium transient decline .
	manualset3
139694	3	407459	5	NULL	NULL	0	NULL	force development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Staurosporine had no frequency-dependent effect on force development , kinetics , calcium transient amplitude , or rate of calcium transient decline .
	manualset3
139695	4	407459	5	NULL	NULL	0	NULL	kinetics 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Staurosporine had no frequency-dependent effect on force development , kinetics , calcium transient amplitude , or rate of calcium transient decline .
	manualset3
139696	5	407459	5	NULL	NULL	0	NULL	calcium transient amplitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Staurosporine had no frequency-dependent effect on force development , kinetics , calcium transient amplitude , or rate of calcium transient decline .
	manualset3
139697	6	407459	5	NULL	NULL	0	NULL	rate 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Staurosporine had no frequency-dependent effect on force development , kinetics , calcium transient amplitude , or rate of calcium transient decline .
	manualset3
139698	7	407459	5	NULL	NULL	0	NULL	calcium transient decline	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Staurosporine had no frequency-dependent effect on force development , kinetics , calcium transient amplitude , or rate of calcium transient decline .
	manualset3
139699	1	407460	5	NULL	NULL	0	NULL	Steady-state analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Steady-state analysis indicated that the Delta45 supported NO synthesis in the absence of CaM at 60 % of the rate in its presence , consistent with our prior result that CaM-bound Delta45 retained 60 % of its activity in the presence of 10 mm EGTA .
	manualset3
139700	2	407460	5	NULL	NULL	0	NULL	Delta45 supported NO synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Steady-state analysis indicated that the Delta45 supported NO synthesis in the absence of CaM at 60 % of the rate in its presence , consistent with our prior result that CaM-bound Delta45 retained 60 % of its activity in the presence of 10 mm EGTA .
	manualset3
139701	3	407460	5	NULL	NULL	0	NULL	absence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Steady-state analysis indicated that the Delta45 supported NO synthesis in the absence of CaM at 60 % of the rate in its presence , consistent with our prior result that CaM-bound Delta45 retained 60 % of its activity in the presence of 10 mm EGTA .
	manualset3
139702	4	407460	5	NULL	NULL	0	NULL	CaM 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Steady-state analysis indicated that the Delta45 supported NO synthesis in the absence of CaM at 60 % of the rate in its presence , consistent with our prior result that CaM-bound Delta45 retained 60 % of its activity in the presence of 10 mm EGTA .
	manualset3
139703	5	407460	5	NULL	NULL	0	NULL	60 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Steady-state analysis indicated that the Delta45 supported NO synthesis in the absence of CaM at 60 % of the rate in its presence , consistent with our prior result that CaM-bound Delta45 retained 60 % of its activity in the presence of 10 mm EGTA .
	manualset3
139704	6	407460	5	NULL	NULL	0	NULL	rate 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Steady-state analysis indicated that the Delta45 supported NO synthesis in the absence of CaM at 60 % of the rate in its presence , consistent with our prior result that CaM-bound Delta45 retained 60 % of its activity in the presence of 10 mm EGTA .
	manualset3
139705	7	407460	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Steady-state analysis indicated that the Delta45 supported NO synthesis in the absence of CaM at 60 % of the rate in its presence , consistent with our prior result that CaM-bound Delta45 retained 60 % of its activity in the presence of 10 mm EGTA .
	manualset3
139706	8	407460	5	NULL	NULL	0	NULL	result 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Steady-state analysis indicated that the Delta45 supported NO synthesis in the absence of CaM at 60 % of the rate in its presence , consistent with our prior result that CaM-bound Delta45 retained 60 % of its activity in the presence of 10 mm EGTA .
	manualset3
139707	9	407460	5	NULL	NULL	0	NULL	CaM-bound Delta45 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Steady-state analysis indicated that the Delta45 supported NO synthesis in the absence of CaM at 60 % of the rate in its presence , consistent with our prior result that CaM-bound Delta45 retained 60 % of its activity in the presence of 10 mm EGTA .
	manualset3
139708	10	407460	5	NULL	NULL	0	NULL	60 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Steady-state analysis indicated that the Delta45 supported NO synthesis in the absence of CaM at 60 % of the rate in its presence , consistent with our prior result that CaM-bound Delta45 retained 60 % of its activity in the presence of 10 mm EGTA .
	manualset3
139709	11	407460	5	NULL	NULL	0	NULL	activity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Steady-state analysis indicated that the Delta45 supported NO synthesis in the absence of CaM at 60 % of the rate in its presence , consistent with our prior result that CaM-bound Delta45 retained 60 % of its activity in the presence of 10 mm EGTA .
	manualset3
139710	12	407460	5	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Steady-state analysis indicated that the Delta45 supported NO synthesis in the absence of CaM at 60 % of the rate in its presence , consistent with our prior result that CaM-bound Delta45 retained 60 % of its activity in the presence of 10 mm EGTA .
	manualset3
139711	13	407460	5	NULL	NULL	0	NULL	10 mm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Steady-state analysis indicated that the Delta45 supported NO synthesis in the absence of CaM at 60 % of the rate in its presence , consistent with our prior result that CaM-bound Delta45 retained 60 % of its activity in the presence of 10 mm EGTA .
	manualset3
139712	14	407460	5	NULL	NULL	0	NULL	EGTA 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Steady-state analysis indicated that the Delta45 supported NO synthesis in the absence of CaM at 60 % of the rate in its presence , consistent with our prior result that CaM-bound Delta45 retained 60 % of its activity in the presence of 10 mm EGTA .
	manualset3
139713	1	407461	5	NULL	NULL	0	NULL	pilot study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A pilot study to evaluate the effect of soy isolate protein on the serum lipid profile and other potential cardiovascular risk markers in moderately hypercholesterolemic chinese adults .
	manualset3
139714	2	407461	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A pilot study to evaluate the effect of soy isolate protein on the serum lipid profile and other potential cardiovascular risk markers in moderately hypercholesterolemic chinese adults .
	manualset3
139715	3	407461	5	NULL	NULL	0	NULL	soy isolate protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A pilot study to evaluate the effect of soy isolate protein on the serum lipid profile and other potential cardiovascular risk markers in moderately hypercholesterolemic chinese adults .
	manualset3
139716	4	407461	5	NULL	NULL	0	NULL	serum lipid profile	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A pilot study to evaluate the effect of soy isolate protein on the serum lipid profile and other potential cardiovascular risk markers in moderately hypercholesterolemic chinese adults .
	manualset3
139717	5	407461	5	NULL	NULL	0	NULL	potential cardiovascular risk markers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A pilot study to evaluate the effect of soy isolate protein on the serum lipid profile and other potential cardiovascular risk markers in moderately hypercholesterolemic chinese adults .
	manualset3
139718	6	407461	5	NULL	NULL	0	NULL	hypercholesterolemic chinese adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A pilot study to evaluate the effect of soy isolate protein on the serum lipid profile and other potential cardiovascular risk markers in moderately hypercholesterolemic chinese adults .
	manualset3
139719	1	407462	5	NULL	NULL	0	NULL	Steady-state kinetics	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Steady-state kinetics reveals substrate cooperativity for SgrAI cleavage on both canonical and secondary sites .
	manualset3
139720	2	407462	5	NULL	NULL	0	NULL	substrate cooperativity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Steady-state kinetics reveals substrate cooperativity for SgrAI cleavage on both canonical and secondary sites .
	manualset3
139721	3	407462	5	NULL	NULL	0	NULL	SgrAI cleavage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Steady-state kinetics reveals substrate cooperativity for SgrAI cleavage on both canonical and secondary sites .
	manualset3
139722	4	407462	5	NULL	NULL	0	NULL	canonical sites 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Steady-state kinetics reveals substrate cooperativity for SgrAI cleavage on both canonical and secondary sites .
	manualset3
139723	5	407462	5	NULL	NULL	0	NULL	secondary sites 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Steady-state kinetics reveals substrate cooperativity for SgrAI cleavage on both canonical and secondary sites .
	manualset3
139724	1	407463	5	NULL	NULL	0	NULL	Steady-state solution 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Steady-state solution of probabilistic gene regulatory networks .
	manualset3
139725	2	407463	5	NULL	NULL	0	NULL	probabilistic gene regulatory networks	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Steady-state solution of probabilistic gene regulatory networks .
	manualset3
139726	1	407464	5	NULL	NULL	0	NULL	Steady states	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Steady states of a nonequilibrium lattice gas .
	manualset3
139727	2	407464	5	NULL	NULL	0	NULL	nonequilibrium lattice gas	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Steady states of a nonequilibrium lattice gas .
	manualset3
139728	1	407465	5	NULL	NULL	0	NULL	Stemofoline 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Stemofoline could increase the accumulation or retention of radiolabeled drugs or fluorescent P-gp substrates in a dose-dependent manner .
	manualset3
139729	2	407465	5	NULL	NULL	0	NULL	accumulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Stemofoline could increase the accumulation or retention of radiolabeled drugs or fluorescent P-gp substrates in a dose-dependent manner .
	manualset3
139730	3	407465	5	NULL	NULL	0	NULL	retention 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Stemofoline could increase the accumulation or retention of radiolabeled drugs or fluorescent P-gp substrates in a dose-dependent manner .
	manualset3
139731	4	407465	5	NULL	NULL	0	NULL	radiolabeled drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Stemofoline could increase the accumulation or retention of radiolabeled drugs or fluorescent P-gp substrates in a dose-dependent manner .
	manualset3
139732	5	407465	5	NULL	NULL	0	NULL	fluorescent P-gp substrates	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stemofoline could increase the accumulation or retention of radiolabeled drugs or fluorescent P-gp substrates in a dose-dependent manner .
	manualset3
139733	6	407465	5	NULL	NULL	0	NULL	dose-dependent manner	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Stemofoline could increase the accumulation or retention of radiolabeled drugs or fluorescent P-gp substrates in a dose-dependent manner .
	manualset3
139734	1	407466	5	NULL	NULL	NULL	NULL	Step-by-step mark-up	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Step-by-step mark-up of medical guideline documents .
	manualset3
139735	2	407466	5	NULL	NULL	0	NULL	medical guideline documents	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Step-by-step mark-up of medical guideline documents .
	manualset3
139736	1	407467	5	NULL	NULL	0	NULL	Stepping stability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Stepping stability : effects of sensory perturbation .
	manualset3
139737	2	407467	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Stepping stability : effects of sensory perturbation .
	manualset3
139738	3	407467	5	NULL	NULL	0	NULL	sensory perturbation	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stepping stability : effects of sensory perturbation .
	manualset3
139739	1	407468	5	NULL	NULL	0	NULL	Stepwise multiple regression analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stepwise multiple regression analysis showed that longer calving to conception intervals were associated with altered profiles of IGF-I , urea and body condition score .
	manualset3
139740	2	407468	5	NULL	NULL	0	NULL	conception intervals	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Stepwise multiple regression analysis showed that longer calving to conception intervals were associated with altered profiles of IGF-I , urea and body condition score .
	manualset3
139741	3	407468	5	NULL	NULL	0	NULL	altered profiles	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Stepwise multiple regression analysis showed that longer calving to conception intervals were associated with altered profiles of IGF-I , urea and body condition score .
	manualset3
139742	4	407468	5	NULL	NULL	0	NULL	 IGF-I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Stepwise multiple regression analysis showed that longer calving to conception intervals were associated with altered profiles of IGF-I , urea and body condition score .
	manualset3
139743	5	407468	5	NULL	NULL	0	NULL	urea 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Stepwise multiple regression analysis showed that longer calving to conception intervals were associated with altered profiles of IGF-I , urea and body condition score .
	manualset3
139744	6	407468	5	NULL	NULL	0	NULL	body condition score	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stepwise multiple regression analysis showed that longer calving to conception intervals were associated with altered profiles of IGF-I , urea and body condition score .
	manualset3
139745	1	407469	5	NULL	NULL	0	NULL	Stepwise regression analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stepwise regression analysis showed a large contribution to the grading was made by the size of the oropharyngeal airway measured by lateral cephalometry .
	manualset3
139746	2	407469	5	NULL	NULL	0	NULL	large contribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Stepwise regression analysis showed a large contribution to the grading was made by the size of the oropharyngeal airway measured by lateral cephalometry .
	manualset3
139747	3	407469	5	NULL	NULL	0	NULL	size 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stepwise regression analysis showed a large contribution to the grading was made by the size of the oropharyngeal airway measured by lateral cephalometry .
	manualset3
139748	4	407469	5	NULL	NULL	0	NULL	oropharyngeal airway 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Stepwise regression analysis showed a large contribution to the grading was made by the size of the oropharyngeal airway measured by lateral cephalometry .
	manualset3
139749	5	407469	5	NULL	NULL	0	NULL	lateral cephalometry	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Stepwise regression analysis showed a large contribution to the grading was made by the size of the oropharyngeal airway measured by lateral cephalometry .
	manualset3
139750	1	407470	5	NULL	NULL	0	NULL	Stereoselective olefin isomerization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stereoselective olefin isomerization leading to asymmetric quaternary carbon construction .
	manualset3
139751	2	407470	5	NULL	NULL	0	NULL	asymmetric quaternary carbon construction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stereoselective olefin isomerization leading to asymmetric quaternary carbon construction .
	manualset3
139752	1	407471	5	NULL	NULL	0	NULL	Stereotypical thinking	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stereotypical thinking about foods and perceived capacity to promote weight gain .
	manualset3
139753	2	407471	5	NULL	NULL	0	NULL	foods 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Stereotypical thinking about foods and perceived capacity to promote weight gain .
	manualset3
139754	3	407471	5	NULL	NULL	0	NULL	perceived capacity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stereotypical thinking about foods and perceived capacity to promote weight gain .
	manualset3
139755	4	407471	5	NULL	NULL	0	NULL	weight gain	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Stereotypical thinking about foods and perceived capacity to promote weight gain .
	manualset3
139756	1	407472	5	NULL	NULL	0	NULL	Steroid eye drops 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Steroid eye drops must be avoided .
	manualset3
139757	1	407473	5	NULL	NULL	0	NULL	Steroids 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Steroids produced a good therapeutic result in most patients ; the remaining patients responded to cromolyn and/or surgery .
	manualset3
139758	2	407473	5	NULL	NULL	0	NULL	therapeutic result	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Steroids produced a good therapeutic result in most patients ; the remaining patients responded to cromolyn and/or surgery .
	manualset3
139759	3	407473	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Steroids produced a good therapeutic result in most patients ; the remaining patients responded to cromolyn and/or surgery .
	manualset3
139760	4	407473	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Steroids produced a good therapeutic result in most patients ; the remaining patients responded to cromolyn and/or surgery .
	manualset3
139761	5	407473	5	NULL	NULL	0	NULL	cromolyn 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Steroids produced a good therapeutic result in most patients ; the remaining patients responded to cromolyn and/or surgery .
	manualset3
139762	6	407473	5	NULL	NULL	0	NULL	surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Steroids produced a good therapeutic result in most patients ; the remaining patients responded to cromolyn and/or surgery .
	manualset3
139763	1	407474	5	NULL	NULL	0	NULL	Sterol 14-demethylase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sterol 14-demethylase from Penicillium digitatum ( PdCYP51 ) is a prime target of antifungal drugs for citrus disease in plants .
	manualset3
139764	2	407474	5	NULL	NULL	0	NULL	Penicillium digitatum ( PdCYP51 )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sterol 14-demethylase from Penicillium digitatum ( PdCYP51 ) is a prime target of antifungal drugs for citrus disease in plants .
	manualset3
139765	3	407474	5	NULL	NULL	0	NULL	prime target	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sterol 14-demethylase from Penicillium digitatum ( PdCYP51 ) is a prime target of antifungal drugs for citrus disease in plants .
	manualset3
139766	4	407474	5	NULL	NULL	0	NULL	antifungal drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Sterol 14-demethylase from Penicillium digitatum ( PdCYP51 ) is a prime target of antifungal drugs for citrus disease in plants .
	manualset3
139767	5	407474	5	NULL	NULL	0	NULL	citrus disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Sterol 14-demethylase from Penicillium digitatum ( PdCYP51 ) is a prime target of antifungal drugs for citrus disease in plants .
	manualset3
139768	6	407474	5	NULL	NULL	0	NULL	plants 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sterol 14-demethylase from Penicillium digitatum ( PdCYP51 ) is a prime target of antifungal drugs for citrus disease in plants .
	manualset3
139769	1	407475	5	NULL	NULL	0	NULL	planar spiral coil 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A planar spiral coil has been used to induce hypersonic evanescent waves in a quartz substrate with the unique ability to focus the acoustic wave down onto the chemical recognition layer .
	manualset3
139770	2	407475	5	NULL	NULL	0	NULL	hypersonic evanescent waves	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A planar spiral coil has been used to induce hypersonic evanescent waves in a quartz substrate with the unique ability to focus the acoustic wave down onto the chemical recognition layer .
	manualset3
139771	3	407475	5	NULL	NULL	0	NULL	quartz substrate 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A planar spiral coil has been used to induce hypersonic evanescent waves in a quartz substrate with the unique ability to focus the acoustic wave down onto the chemical recognition layer .
	manualset3
139772	4	407475	5	NULL	NULL	0	NULL	unique ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A planar spiral coil has been used to induce hypersonic evanescent waves in a quartz substrate with the unique ability to focus the acoustic wave down onto the chemical recognition layer .
	manualset3
139773	5	407475	5	NULL	NULL	0	NULL	focus 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A planar spiral coil has been used to induce hypersonic evanescent waves in a quartz substrate with the unique ability to focus the acoustic wave down onto the chemical recognition layer .
	manualset3
139774	6	407475	5	NULL	NULL	0	NULL	acoustic wave 	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A planar spiral coil has been used to induce hypersonic evanescent waves in a quartz substrate with the unique ability to focus the acoustic wave down onto the chemical recognition layer .
	manualset3
139775	7	407475	5	NULL	NULL	0	NULL	chemical recognition layer	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A planar spiral coil has been used to induce hypersonic evanescent waves in a quartz substrate with the unique ability to focus the acoustic wave down onto the chemical recognition layer .
	manualset3
139776	1	407476	5	NULL	NULL	0	NULL	positive phototaxis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Still , positive phototaxis is the only behavior described so far that is likely to be correlated with the eyes .
	manualset3
139777	2	407476	5	NULL	NULL	0	NULL	behavior 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Still , positive phototaxis is the only behavior described so far that is likely to be correlated with the eyes .
	manualset3
139778	3	407476	5	NULL	NULL	0	NULL	eyes 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Still , positive phototaxis is the only behavior described so far that is likely to be correlated with the eyes .
	manualset3
139779	1	407477	5	NULL	NULL	0	NULL	Stim 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Stim senses depletion of the ER Ca ( 2 + ) store and physically relays this information by translocating from the ER to junctions adjacent to the plasma membrane , and Orai embodies the pore of the plasma membrane calcium channel .
	manualset3
139780	2	407477	5	NULL	NULL	0	NULL	depletion 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stim senses depletion of the ER Ca ( 2 + ) store and physically relays this information by translocating from the ER to junctions adjacent to the plasma membrane , and Orai embodies the pore of the plasma membrane calcium channel .
	manualset3
139781	3	407477	5	NULL	NULL	0	NULL	ER Ca ( 2 + ) store	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Stim senses depletion of the ER Ca ( 2 + ) store and physically relays this information by translocating from the ER to junctions adjacent to the plasma membrane , and Orai embodies the pore of the plasma membrane calcium channel .
	manualset3
139782	4	407477	5	NULL	NULL	0	NULL	information 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Stim senses depletion of the ER Ca ( 2 + ) store and physically relays this information by translocating from the ER to junctions adjacent to the plasma membrane , and Orai embodies the pore of the plasma membrane calcium channel .
	manualset3
139783	5	407477	5	NULL	NULL	0	NULL	ER 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Stim senses depletion of the ER Ca ( 2 + ) store and physically relays this information by translocating from the ER to junctions adjacent to the plasma membrane , and Orai embodies the pore of the plasma membrane calcium channel .
	manualset3
139784	6	407477	5	NULL	NULL	0	NULL	junctions adjacent to the plasma membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Stim senses depletion of the ER Ca ( 2 + ) store and physically relays this information by translocating from the ER to junctions adjacent to the plasma membrane , and Orai embodies the pore of the plasma membrane calcium channel .
	manualset3
139785	7	407477	5	NULL	NULL	0	NULL	Orai 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Stim senses depletion of the ER Ca ( 2 + ) store and physically relays this information by translocating from the ER to junctions adjacent to the plasma membrane , and Orai embodies the pore of the plasma membrane calcium channel .
	manualset3
139786	8	407477	5	NULL	NULL	0	NULL	pore 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Stim senses depletion of the ER Ca ( 2 + ) store and physically relays this information by translocating from the ER to junctions adjacent to the plasma membrane , and Orai embodies the pore of the plasma membrane calcium channel .
	manualset3
139787	9	407477	5	NULL	NULL	0	NULL	plasma membrane calcium channel	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Stim senses depletion of the ER Ca ( 2 + ) store and physically relays this information by translocating from the ER to junctions adjacent to the plasma membrane , and Orai embodies the pore of the plasma membrane calcium channel .
	manualset3
139788	1	407478	5	NULL	NULL	0	NULL	Stimulated secretion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulated secretion was dependent on calcium and temperature , and could be elicited from NSS maintained in culture for 4 days .
	manualset3
139789	2	407478	5	NULL	NULL	0	NULL	calcium 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulated secretion was dependent on calcium and temperature , and could be elicited from NSS maintained in culture for 4 days .
	manualset3
139790	3	407478	5	NULL	NULL	0	NULL	temperature 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulated secretion was dependent on calcium and temperature , and could be elicited from NSS maintained in culture for 4 days .
	manualset3
139791	4	407478	5	NULL	NULL	0	NULL	NSS 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulated secretion was dependent on calcium and temperature , and could be elicited from NSS maintained in culture for 4 days .
	manualset3
139792	5	407478	5	NULL	NULL	0	NULL	culture 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulated secretion was dependent on calcium and temperature , and could be elicited from NSS maintained in culture for 4 days .
	manualset3
139793	6	407478	5	NULL	NULL	0	NULL	4 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulated secretion was dependent on calcium and temperature , and could be elicited from NSS maintained in culture for 4 days .
	manualset3
139794	1	407479	5	NULL	NULL	0	NULL	plea 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A plea is made in this paper to remove the prostate under direct vision by a retropubic route rather than by attempting a blind suprapubic ( transvesical ) procedure .
	manualset3
139795	2	407479	5	NULL	NULL	0	NULL	paper 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A plea is made in this paper to remove the prostate under direct vision by a retropubic route rather than by attempting a blind suprapubic ( transvesical ) procedure .
	manualset3
139796	3	407479	5	NULL	NULL	0	NULL	prostate 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A plea is made in this paper to remove the prostate under direct vision by a retropubic route rather than by attempting a blind suprapubic ( transvesical ) procedure .
	manualset3
139797	4	407479	5	NULL	NULL	0	NULL	direct vision 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A plea is made in this paper to remove the prostate under direct vision by a retropubic route rather than by attempting a blind suprapubic ( transvesical ) procedure .
	manualset3
139798	5	407479	5	NULL	NULL	0	NULL	retropubic route 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A plea is made in this paper to remove the prostate under direct vision by a retropubic route rather than by attempting a blind suprapubic ( transvesical ) procedure .
	manualset3
139799	6	407479	5	NULL	NULL	0	NULL	blind suprapubic ( transvesical ) procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A plea is made in this paper to remove the prostate under direct vision by a retropubic route rather than by attempting a blind suprapubic ( transvesical ) procedure .
	manualset3
139800	1	407480	5	NULL	NULL	0	NULL	supernatants 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulated and control supernatants were placed on the attractant side of cellulose ester filters with normal human monocytes as responder cells .
	manualset3
139801	2	407480	5	NULL	NULL	0	NULL	attractant side	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulated and control supernatants were placed on the attractant side of cellulose ester filters with normal human monocytes as responder cells .
	manualset3
139802	3	407480	5	NULL	NULL	0	NULL	cellulose ester filters	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulated and control supernatants were placed on the attractant side of cellulose ester filters with normal human monocytes as responder cells .
	manualset3
139803	4	407480	5	NULL	NULL	0	NULL	normal human monocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulated and control supernatants were placed on the attractant side of cellulose ester filters with normal human monocytes as responder cells .
	manualset3
139804	5	407480	5	NULL	NULL	0	NULL	responder cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulated and control supernatants were placed on the attractant side of cellulose ester filters with normal human monocytes as responder cells .
	manualset3
139805	1	407481	5	NULL	NULL	0	NULL	Stimulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation and inhibition of neutrophil chemotaxis by endothelin-3 .
	manualset3
139806	2	407481	5	NULL	NULL	0	NULL	inhibition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation and inhibition of neutrophil chemotaxis by endothelin-3 .
	manualset3
139807	3	407481	5	NULL	NULL	0	NULL	neutrophil chemotaxis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation and inhibition of neutrophil chemotaxis by endothelin-3 .
	manualset3
139808	4	407481	5	NULL	NULL	0	NULL	endothelin-3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation and inhibition of neutrophil chemotaxis by endothelin-3 .
	manualset3
139809	1	407482	5	NULL	NULL	0	NULL	Stimulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of G protein-coupled receptor ( GPCR ) results in uniform cell enlargement in all directions with an increase in skeletal alpha-actin ( alpha-SKA ) gene expression , while stimulation of gp130 receptor by interleukin-6 ( IL-6 ) - related cytokines induces longitudinal elongation with no increase in alpha-SKA gene expression .
	manualset3
139810	2	407482	5	NULL	NULL	0	NULL	G protein-coupled receptor ( GPCR )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of G protein-coupled receptor ( GPCR ) results in uniform cell enlargement in all directions with an increase in skeletal alpha-actin ( alpha-SKA ) gene expression , while stimulation of gp130 receptor by interleukin-6 ( IL-6 ) - related cytokines induces longitudinal elongation with no increase in alpha-SKA gene expression .
	manualset3
139811	3	407482	5	NULL	NULL	0	NULL	uniform cell enlargement	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of G protein-coupled receptor ( GPCR ) results in uniform cell enlargement in all directions with an increase in skeletal alpha-actin ( alpha-SKA ) gene expression , while stimulation of gp130 receptor by interleukin-6 ( IL-6 ) - related cytokines induces longitudinal elongation with no increase in alpha-SKA gene expression .
	manualset3
139812	4	407482	5	NULL	NULL	0	NULL	directions 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of G protein-coupled receptor ( GPCR ) results in uniform cell enlargement in all directions with an increase in skeletal alpha-actin ( alpha-SKA ) gene expression , while stimulation of gp130 receptor by interleukin-6 ( IL-6 ) - related cytokines induces longitudinal elongation with no increase in alpha-SKA gene expression .
	manualset3
139813	5	407482	5	NULL	NULL	0	NULL	skeletal alpha-actin ( alpha-SKA ) gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of G protein-coupled receptor ( GPCR ) results in uniform cell enlargement in all directions with an increase in skeletal alpha-actin ( alpha-SKA ) gene expression , while stimulation of gp130 receptor by interleukin-6 ( IL-6 ) - related cytokines induces longitudinal elongation with no increase in alpha-SKA gene expression .
	manualset3
139814	6	407482	5	NULL	NULL	0	NULL	stimulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of G protein-coupled receptor ( GPCR ) results in uniform cell enlargement in all directions with an increase in skeletal alpha-actin ( alpha-SKA ) gene expression , while stimulation of gp130 receptor by interleukin-6 ( IL-6 ) - related cytokines induces longitudinal elongation with no increase in alpha-SKA gene expression .
	manualset3
139815	7	407482	5	NULL	NULL	0	NULL	 gp130 receptor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of G protein-coupled receptor ( GPCR ) results in uniform cell enlargement in all directions with an increase in skeletal alpha-actin ( alpha-SKA ) gene expression , while stimulation of gp130 receptor by interleukin-6 ( IL-6 ) - related cytokines induces longitudinal elongation with no increase in alpha-SKA gene expression .
	manualset3
139816	8	407482	5	NULL	NULL	0	NULL	interleukin-6 ( IL-6 ) - related cytokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of G protein-coupled receptor ( GPCR ) results in uniform cell enlargement in all directions with an increase in skeletal alpha-actin ( alpha-SKA ) gene expression , while stimulation of gp130 receptor by interleukin-6 ( IL-6 ) - related cytokines induces longitudinal elongation with no increase in alpha-SKA gene expression .
	manualset3
139817	9	407482	5	NULL	NULL	0	NULL	longitudinal elongation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of G protein-coupled receptor ( GPCR ) results in uniform cell enlargement in all directions with an increase in skeletal alpha-actin ( alpha-SKA ) gene expression , while stimulation of gp130 receptor by interleukin-6 ( IL-6 ) - related cytokines induces longitudinal elongation with no increase in alpha-SKA gene expression .
	manualset3
139818	10	407482	5	NULL	NULL	0	NULL	alpha-SKA gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of G protein-coupled receptor ( GPCR ) results in uniform cell enlargement in all directions with an increase in skeletal alpha-actin ( alpha-SKA ) gene expression , while stimulation of gp130 receptor by interleukin-6 ( IL-6 ) - related cytokines induces longitudinal elongation with no increase in alpha-SKA gene expression .
	manualset3
139819	1	407483	5	NULL	NULL	0	NULL	Stimulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of angiotensin II AT1 receptors in rat median eminence increases phosphoinositide hydrolysis .
	manualset3
139820	2	407483	5	NULL	NULL	0	NULL	angiotensin II AT1 receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of angiotensin II AT1 receptors in rat median eminence increases phosphoinositide hydrolysis .
	manualset3
139821	3	407483	5	NULL	NULL	0	NULL	rat median eminence	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of angiotensin II AT1 receptors in rat median eminence increases phosphoinositide hydrolysis .
	manualset3
139822	4	407483	5	NULL	NULL	0	NULL	phosphoinositide hydrolysis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of angiotensin II AT1 receptors in rat median eminence increases phosphoinositide hydrolysis .
	manualset3
139823	1	407484	5	NULL	NULL	0	NULL	Stimulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of cephalosporin production by methionine peptides in a mutant blocked in reverse transsulfuration .
	manualset3
139824	2	407484	5	NULL	NULL	0	NULL	cephalosporin production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of cephalosporin production by methionine peptides in a mutant blocked in reverse transsulfuration .
	manualset3
139825	3	407484	5	NULL	NULL	0	NULL	methionine peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of cephalosporin production by methionine peptides in a mutant blocked in reverse transsulfuration .
	manualset3
139826	4	407484	5	NULL	NULL	0	NULL	mutant 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of cephalosporin production by methionine peptides in a mutant blocked in reverse transsulfuration .
	manualset3
139827	5	407484	5	NULL	NULL	0	NULL	reverse transsulfuration	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of cephalosporin production by methionine peptides in a mutant blocked in reverse transsulfuration .
	manualset3
139828	1	407485	5	NULL	NULL	0	NULL	Stimulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of chick retinal ganglioside synthesis by light .
	manualset3
139829	2	407485	5	NULL	NULL	0	NULL	chick retinal ganglioside synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of chick retinal ganglioside synthesis by light .
	manualset3
139830	3	407485	5	NULL	NULL	0	NULL	light 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of chick retinal ganglioside synthesis by light .
	manualset3
139831	1	407486	5	NULL	NULL	0	NULL	Stimulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of human hemopoietic cells by colony stimulating factors : sensitivity of leukemia cells .
	manualset3
139832	2	407486	5	NULL	NULL	0	NULL	human hemopoietic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of human hemopoietic cells by colony stimulating factors : sensitivity of leukemia cells .
	manualset3
139833	3	407486	5	NULL	NULL	0	NULL	colony stimulating factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of human hemopoietic cells by colony stimulating factors : sensitivity of leukemia cells .
	manualset3
139834	4	407486	5	NULL	NULL	0	NULL	sensitivity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of human hemopoietic cells by colony stimulating factors : sensitivity of leukemia cells .
	manualset3
139835	5	407486	5	NULL	NULL	0	NULL	leukemia cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of human hemopoietic cells by colony stimulating factors : sensitivity of leukemia cells .
	manualset3
139836	1	407487	5	NULL	NULL	NULL	NULL	Stimulation 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Stimulation of interstitial cell growth after selective destruction of foetal Leydig cells in the testis of postnatal rats .
	manualset3
139837	2	407487	5	NULL	NULL	0	NULL	interstitial cell growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of interstitial cell growth after selective destruction of foetal Leydig cells in the testis of postnatal rats .
	manualset3
139838	3	407487	5	NULL	NULL	0	NULL	selective destruction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of interstitial cell growth after selective destruction of foetal Leydig cells in the testis of postnatal rats .
	manualset3
139839	4	407487	5	NULL	NULL	0	NULL	foetal Leydig cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of interstitial cell growth after selective destruction of foetal Leydig cells in the testis of postnatal rats .
	manualset3
139840	5	407487	5	NULL	NULL	0	NULL	testis 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of interstitial cell growth after selective destruction of foetal Leydig cells in the testis of postnatal rats .
	manualset3
139841	6	407487	5	NULL	NULL	0	NULL	postnatal rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of interstitial cell growth after selective destruction of foetal Leydig cells in the testis of postnatal rats .
	manualset3
139842	1	407488	5	NULL	NULL	0	NULL	Stimulation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of lamellipodium extension by concanavalin A is inhibited by low temperature ( 4 degrees C ) , 2 , 4-dinitrophenol ( 0.2 mM ) , cytochalasin D ( 4 microM ) , or trifluoperazine ( 10 microM ) , but not by cycloheximide ( 360 microM ) or colchicine ( 12.5 microM ) .
	manualset3
139843	2	407488	5	NULL	NULL	0	NULL	lamellipodium extension	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of lamellipodium extension by concanavalin A is inhibited by low temperature ( 4 degrees C ) , 2 , 4-dinitrophenol ( 0.2 mM ) , cytochalasin D ( 4 microM ) , or trifluoperazine ( 10 microM ) , but not by cycloheximide ( 360 microM ) or colchicine ( 12.5 microM ) .
	manualset3
139844	3	407488	5	NULL	NULL	0	NULL	concanavalin A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of lamellipodium extension by concanavalin A is inhibited by low temperature ( 4 degrees C ) , 2 , 4-dinitrophenol ( 0.2 mM ) , cytochalasin D ( 4 microM ) , or trifluoperazine ( 10 microM ) , but not by cycloheximide ( 360 microM ) or colchicine ( 12.5 microM ) .
	manualset3
139845	4	407488	5	NULL	NULL	0	NULL	low temperature 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of lamellipodium extension by concanavalin A is inhibited by low temperature ( 4 degrees C ) , 2 , 4-dinitrophenol ( 0.2 mM ) , cytochalasin D ( 4 microM ) , or trifluoperazine ( 10 microM ) , but not by cycloheximide ( 360 microM ) or colchicine ( 12.5 microM ) .
	manualset3
139846	5	407488	5	NULL	NULL	0	NULL	 4 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of lamellipodium extension by concanavalin A is inhibited by low temperature ( 4 degrees C ) , 2 , 4-dinitrophenol ( 0.2 mM ) , cytochalasin D ( 4 microM ) , or trifluoperazine ( 10 microM ) , but not by cycloheximide ( 360 microM ) or colchicine ( 12.5 microM ) .
	manualset3
139847	6	407488	5	NULL	NULL	0	NULL	2 , 4-dinitrophenol 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of lamellipodium extension by concanavalin A is inhibited by low temperature ( 4 degrees C ) , 2 , 4-dinitrophenol ( 0.2 mM ) , cytochalasin D ( 4 microM ) , or trifluoperazine ( 10 microM ) , but not by cycloheximide ( 360 microM ) or colchicine ( 12.5 microM ) .
	manualset3
139848	7	407488	5	NULL	NULL	0	NULL	0.2 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of lamellipodium extension by concanavalin A is inhibited by low temperature ( 4 degrees C ) , 2 , 4-dinitrophenol ( 0.2 mM ) , cytochalasin D ( 4 microM ) , or trifluoperazine ( 10 microM ) , but not by cycloheximide ( 360 microM ) or colchicine ( 12.5 microM ) .
	manualset3
139849	8	407488	5	NULL	NULL	0	NULL	cytochalasin D	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of lamellipodium extension by concanavalin A is inhibited by low temperature ( 4 degrees C ) , 2 , 4-dinitrophenol ( 0.2 mM ) , cytochalasin D ( 4 microM ) , or trifluoperazine ( 10 microM ) , but not by cycloheximide ( 360 microM ) or colchicine ( 12.5 microM ) .
	manualset3
139850	9	407488	5	NULL	NULL	0	NULL	4 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of lamellipodium extension by concanavalin A is inhibited by low temperature ( 4 degrees C ) , 2 , 4-dinitrophenol ( 0.2 mM ) , cytochalasin D ( 4 microM ) , or trifluoperazine ( 10 microM ) , but not by cycloheximide ( 360 microM ) or colchicine ( 12.5 microM ) .
	manualset3
139851	10	407488	5	NULL	NULL	0	NULL	trifluoperazine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of lamellipodium extension by concanavalin A is inhibited by low temperature ( 4 degrees C ) , 2 , 4-dinitrophenol ( 0.2 mM ) , cytochalasin D ( 4 microM ) , or trifluoperazine ( 10 microM ) , but not by cycloheximide ( 360 microM ) or colchicine ( 12.5 microM ) .
	manualset3
139852	11	407488	5	NULL	NULL	0	NULL	10 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of lamellipodium extension by concanavalin A is inhibited by low temperature ( 4 degrees C ) , 2 , 4-dinitrophenol ( 0.2 mM ) , cytochalasin D ( 4 microM ) , or trifluoperazine ( 10 microM ) , but not by cycloheximide ( 360 microM ) or colchicine ( 12.5 microM ) .
	manualset3
139853	12	407488	5	NULL	NULL	0	NULL	cycloheximide 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of lamellipodium extension by concanavalin A is inhibited by low temperature ( 4 degrees C ) , 2 , 4-dinitrophenol ( 0.2 mM ) , cytochalasin D ( 4 microM ) , or trifluoperazine ( 10 microM ) , but not by cycloheximide ( 360 microM ) or colchicine ( 12.5 microM ) .
	manualset3
139854	13	407488	5	NULL	NULL	0	NULL	360 microM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of lamellipodium extension by concanavalin A is inhibited by low temperature ( 4 degrees C ) , 2 , 4-dinitrophenol ( 0.2 mM ) , cytochalasin D ( 4 microM ) , or trifluoperazine ( 10 microM ) , but not by cycloheximide ( 360 microM ) or colchicine ( 12.5 microM ) .
	manualset3
139855	14	407488	5	NULL	NULL	0	NULL	colchicine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of lamellipodium extension by concanavalin A is inhibited by low temperature ( 4 degrees C ) , 2 , 4-dinitrophenol ( 0.2 mM ) , cytochalasin D ( 4 microM ) , or trifluoperazine ( 10 microM ) , but not by cycloheximide ( 360 microM ) or colchicine ( 12.5 microM ) .
	manualset3
139856	15	407488	5	NULL	NULL	0	NULL	12.5 microM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of lamellipodium extension by concanavalin A is inhibited by low temperature ( 4 degrees C ) , 2 , 4-dinitrophenol ( 0.2 mM ) , cytochalasin D ( 4 microM ) , or trifluoperazine ( 10 microM ) , but not by cycloheximide ( 360 microM ) or colchicine ( 12.5 microM ) .
	manualset3
139857	1	407489	5	NULL	NULL	0	NULL	Stimulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of microsomal prostaglandin synthesis by a blood plasma constituent which augments autoregulation and maintenance of vascular tone in isolated rabbit hearts .
	manualset3
139858	2	407489	5	NULL	NULL	0	NULL	microsomal prostaglandin synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of microsomal prostaglandin synthesis by a blood plasma constituent which augments autoregulation and maintenance of vascular tone in isolated rabbit hearts .
	manualset3
139859	3	407489	5	NULL	NULL	0	NULL	blood plasma constituent	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of microsomal prostaglandin synthesis by a blood plasma constituent which augments autoregulation and maintenance of vascular tone in isolated rabbit hearts .
	manualset3
139860	4	407489	5	NULL	NULL	0	NULL	autoregulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of microsomal prostaglandin synthesis by a blood plasma constituent which augments autoregulation and maintenance of vascular tone in isolated rabbit hearts .
	manualset3
139861	5	407489	5	NULL	NULL	0	NULL	maintenance 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of microsomal prostaglandin synthesis by a blood plasma constituent which augments autoregulation and maintenance of vascular tone in isolated rabbit hearts .
	manualset3
139862	6	407489	5	NULL	NULL	0	NULL	vascular tone	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of microsomal prostaglandin synthesis by a blood plasma constituent which augments autoregulation and maintenance of vascular tone in isolated rabbit hearts .
	manualset3
139863	7	407489	5	NULL	NULL	0	NULL	rabbit hearts 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of microsomal prostaglandin synthesis by a blood plasma constituent which augments autoregulation and maintenance of vascular tone in isolated rabbit hearts .
	manualset3
139864	1	407490	5	NULL	NULL	0	NULL	plea 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A plea is made to delineate unknown genesis syndromes with craniosynostosis as rapidly as possible .
	manualset3
139865	2	407490	5	NULL	NULL	0	NULL	unknown genesis syndromes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A plea is made to delineate unknown genesis syndromes with craniosynostosis as rapidly as possible .
	manualset3
139866	3	407490	5	NULL	NULL	0	NULL	craniosynostosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A plea is made to delineate unknown genesis syndromes with craniosynostosis as rapidly as possible .
	manualset3
139867	1	407491	5	NULL	NULL	0	NULL	Stimulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of the immune system could possible be obtained using dendritic cells cultured in vitro and loaded with tumor antigens .
	manualset3
139868	2	407491	5	NULL	NULL	0	NULL	immune system	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of the immune system could possible be obtained using dendritic cells cultured in vitro and loaded with tumor antigens .
	manualset3
139869	3	407491	5	NULL	NULL	0	NULL	dendritic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of the immune system could possible be obtained using dendritic cells cultured in vitro and loaded with tumor antigens .
	manualset3
139870	4	407491	5	NULL	NULL	0	NULL	tumor antigens	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of the immune system could possible be obtained using dendritic cells cultured in vitro and loaded with tumor antigens .
	manualset3
139871	1	407492	5	NULL	NULL	0	NULL	Stimulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of the posterior hypothalamic nucleus was less effective in this respect .
	manualset3
139872	2	407492	5	NULL	NULL	0	NULL	posterior hypothalamic nucleus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of the posterior hypothalamic nucleus was less effective in this respect .
	manualset3
139873	1	407493	5	NULL	NULL	0	NULL	Stimuli-responsive multifunctional membranes 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimuli-responsive multifunctional membranes of controllable morphology from poly ( vinylidene fluoride ) - graft-poly ( 2 - ( N , N-dimethylamino ) ethyl methacrylate ) prepared via atom transfer radical polymerization .
	manualset3
139874	2	407493	5	NULL	NULL	0	NULL	morphology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimuli-responsive multifunctional membranes of controllable morphology from poly ( vinylidene fluoride ) - graft-poly ( 2 - ( N , N-dimethylamino ) ethyl methacrylate ) prepared via atom transfer radical polymerization .
	manualset3
139875	3	407493	5	NULL	NULL	0	NULL	poly ( vinylidene fluoride ) - graft-poly ( 2 - ( N , N-dimethylamino ) ethyl methacrylate ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimuli-responsive multifunctional membranes of controllable morphology from poly ( vinylidene fluoride ) - graft-poly ( 2 - ( N , N-dimethylamino ) ethyl methacrylate ) prepared via atom transfer radical polymerization .
	manualset3
139876	4	407493	5	NULL	NULL	0	NULL	atom transfer radical polymerization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimuli-responsive multifunctional membranes of controllable morphology from poly ( vinylidene fluoride ) - graft-poly ( 2 - ( N , N-dimethylamino ) ethyl methacrylate ) prepared via atom transfer radical polymerization .
	manualset3
139877	1	407494	5	NULL	NULL	0	NULL	Stimulus quality	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulus quality in the degraded viewing condition was manipulated by a spatial filtering process .
	manualset3
139878	2	407494	5	NULL	NULL	0	NULL	degraded viewing condition	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulus quality in the degraded viewing condition was manipulated by a spatial filtering process .
	manualset3
139879	3	407494	5	NULL	NULL	0	NULL	spatial filtering process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulus quality in the degraded viewing condition was manipulated by a spatial filtering process .
	manualset3
139880	1	407495	5	NULL	NULL	0	NULL	Stopped-flow kinetics studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stopped-flow kinetics studies suggested at least two distinct kinetic steps for the binding of curcumin to BSA .
	manualset3
139881	2	407495	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Stopped-flow kinetics studies suggested at least two distinct kinetic steps for the binding of curcumin to BSA .
	manualset3
139882	3	407495	5	NULL	NULL	0	NULL	kinetic steps	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Stopped-flow kinetics studies suggested at least two distinct kinetic steps for the binding of curcumin to BSA .
	manualset3
139883	4	407495	5	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stopped-flow kinetics studies suggested at least two distinct kinetic steps for the binding of curcumin to BSA .
	manualset3
139884	5	407495	5	NULL	NULL	0	NULL	curcumin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Stopped-flow kinetics studies suggested at least two distinct kinetic steps for the binding of curcumin to BSA .
	manualset3
139885	6	407495	5	NULL	NULL	0	NULL	BSA 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Stopped-flow kinetics studies suggested at least two distinct kinetic steps for the binding of curcumin to BSA .
	manualset3
139886	1	407496	5	NULL	NULL	0	NULL	smoking 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Stopping smoking reduces the risk of lung cancer and many other cancers , cardiovascular disease , stroke , peripheral vascular disease .
	manualset3
139887	2	407496	5	NULL	NULL	0	NULL	risk 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Stopping smoking reduces the risk of lung cancer and many other cancers , cardiovascular disease , stroke , peripheral vascular disease .
	manualset3
139888	3	407496	5	NULL	NULL	0	NULL	lung cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Stopping smoking reduces the risk of lung cancer and many other cancers , cardiovascular disease , stroke , peripheral vascular disease .
	manualset3
139889	4	407496	5	NULL	NULL	0	NULL	cancers 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Stopping smoking reduces the risk of lung cancer and many other cancers , cardiovascular disease , stroke , peripheral vascular disease .
	manualset3
139890	5	407496	5	NULL	NULL	0	NULL	cardiovascular disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Stopping smoking reduces the risk of lung cancer and many other cancers , cardiovascular disease , stroke , peripheral vascular disease .
	manualset3
139891	6	407496	5	NULL	NULL	NULL	NULL	stroke 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Stopping smoking reduces the risk of lung cancer and many other cancers , cardiovascular disease , stroke , peripheral vascular disease .
	manualset3
139892	7	407496	5	NULL	NULL	0	NULL	peripheral vascular disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Stopping smoking reduces the risk of lung cancer and many other cancers , cardiovascular disease , stroke , peripheral vascular disease .
	manualset3
139893	1	407497	5	NULL	NULL	0	NULL	therapy compliance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A plus for therapy compliance ) .
	manualset3
139894	1	407498	5	NULL	NULL	0	NULL	Storage 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Storage at 4 C for 50 days resulted in approximately 90 % recovery of nematode eggs .
	manualset3
139895	2	407498	5	NULL	NULL	0	NULL	4 C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Storage at 4 C for 50 days resulted in approximately 90 % recovery of nematode eggs .
	manualset3
139896	3	407498	5	NULL	NULL	0	NULL	50 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Storage at 4 C for 50 days resulted in approximately 90 % recovery of nematode eggs .
	manualset3
139897	4	407498	5	NULL	NULL	0	NULL	90 % recovery 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Storage at 4 C for 50 days resulted in approximately 90 % recovery of nematode eggs .
	manualset3
139898	5	407498	5	NULL	NULL	0	NULL	nematode eggs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Storage at 4 C for 50 days resulted in approximately 90 % recovery of nematode eggs .
	manualset3
139899	1	407499	5	NULL	NULL	0	NULL	Storage media	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Storage media did not significantly ( p & gt ; 0.05 ) affect bond durability .
	manualset3
139900	2	407499	5	NULL	NULL	0	NULL	p & gt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Storage media did not significantly ( p & gt ; 0.05 ) affect bond durability .
	manualset3
139901	3	407499	5	NULL	NULL	0	NULL	bond durability 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Storage media did not significantly ( p & gt ; 0.05 ) affect bond durability .
	manualset3
139902	1	407500	5	NULL	NULL	0	NULL	reversal 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Straightening or reversal of cervical lordosis occurred in 29.4 % of patients with goitre and only 8 % of controls , with none of the control group showing reversal of cervical curvature .
	manualset3
139903	2	407500	5	NULL	NULL	0	NULL	cervical lordosis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Straightening or reversal of cervical lordosis occurred in 29.4 % of patients with goitre and only 8 % of controls , with none of the control group showing reversal of cervical curvature .
	manualset3
139904	3	407500	5	NULL	NULL	0	NULL	29.4 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Straightening or reversal of cervical lordosis occurred in 29.4 % of patients with goitre and only 8 % of controls , with none of the control group showing reversal of cervical curvature .
	manualset3
139905	4	407500	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Straightening or reversal of cervical lordosis occurred in 29.4 % of patients with goitre and only 8 % of controls , with none of the control group showing reversal of cervical curvature .
	manualset3
139906	5	407500	5	NULL	NULL	0	NULL	goitre 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Straightening or reversal of cervical lordosis occurred in 29.4 % of patients with goitre and only 8 % of controls , with none of the control group showing reversal of cervical curvature .
	manualset3
139907	6	407500	5	NULL	NULL	0	NULL	8 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Straightening or reversal of cervical lordosis occurred in 29.4 % of patients with goitre and only 8 % of controls , with none of the control group showing reversal of cervical curvature .
	manualset3
139908	7	407500	5	NULL	NULL	0	NULL	controls 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Straightening or reversal of cervical lordosis occurred in 29.4 % of patients with goitre and only 8 % of controls , with none of the control group showing reversal of cervical curvature .
	manualset3
139909	8	407500	5	NULL	NULL	0	NULL	control group 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Straightening or reversal of cervical lordosis occurred in 29.4 % of patients with goitre and only 8 % of controls , with none of the control group showing reversal of cervical curvature .
	manualset3
139910	9	407500	5	NULL	NULL	0	NULL	reversal 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Straightening or reversal of cervical lordosis occurred in 29.4 % of patients with goitre and only 8 % of controls , with none of the control group showing reversal of cervical curvature .
	manualset3
139911	10	407500	5	NULL	NULL	0	NULL	cervical curvature	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Straightening or reversal of cervical lordosis occurred in 29.4 % of patients with goitre and only 8 % of controls , with none of the control group showing reversal of cervical curvature .
	manualset3
139912	1	407501	5	NULL	NULL	0	NULL	Strains 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains producing discrepant results between conventional methods and ITS sequence analysis were analyzed further by sequencing the D1-D2 domain of the large-subunit rRNA gene for species clarification .
	manualset3
139913	2	407501	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains producing discrepant results between conventional methods and ITS sequence analysis were analyzed further by sequencing the D1-D2 domain of the large-subunit rRNA gene for species clarification .
	manualset3
139914	3	407501	5	NULL	NULL	0	NULL	conventional methods 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains producing discrepant results between conventional methods and ITS sequence analysis were analyzed further by sequencing the D1-D2 domain of the large-subunit rRNA gene for species clarification .
	manualset3
139915	4	407501	5	NULL	NULL	0	NULL	ITS sequence analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains producing discrepant results between conventional methods and ITS sequence analysis were analyzed further by sequencing the D1-D2 domain of the large-subunit rRNA gene for species clarification .
	manualset3
139916	5	407501	5	NULL	NULL	0	NULL	D1-D2 domain 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains producing discrepant results between conventional methods and ITS sequence analysis were analyzed further by sequencing the D1-D2 domain of the large-subunit rRNA gene for species clarification .
	manualset3
139917	6	407501	5	NULL	NULL	0	NULL	large-subunit rRNA gene	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains producing discrepant results between conventional methods and ITS sequence analysis were analyzed further by sequencing the D1-D2 domain of the large-subunit rRNA gene for species clarification .
	manualset3
139918	7	407501	5	NULL	NULL	0	NULL	species clarification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains producing discrepant results between conventional methods and ITS sequence analysis were analyzed further by sequencing the D1-D2 domain of the large-subunit rRNA gene for species clarification .
	manualset3
139919	1	407502	5	NULL	NULL	NULL	NULL	Strains 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Strains were constructed in which Hex6-tagged versions of subunits d , OSCP , and b were coexpressed with the corresponding wild-type subunit .
	manualset3
139920	2	407502	5	NULL	NULL	NULL	NULL	Hex6-tagged versions of subunit d 	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Strains were constructed in which Hex6-tagged versions of subunits d , OSCP , and b were coexpressed with the corresponding wild-type subunit .
	manualset3
139921	3	407502	5	NULL	NULL	0	NULL	Hex6-tagged versions of subunits OSCP 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains were constructed in which Hex6-tagged versions of subunits d , OSCP , and b were coexpressed with the corresponding wild-type subunit .
	manualset3
139922	4	407502	5	NULL	NULL	0	NULL	 \tHex6-tagged versions of subunit b	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains were constructed in which Hex6-tagged versions of subunits d , OSCP , and b were coexpressed with the corresponding wild-type subunit .
	manualset3
139923	5	407502	5	NULL	NULL	0	NULL	wild-type subunit	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains were constructed in which Hex6-tagged versions of subunits d , OSCP , and b were coexpressed with the corresponding wild-type subunit .
	manualset3
139924	1	407503	5	NULL	NULL	0	NULL	Strains 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains with enhanced tolerance to other stresses such as heat , fermentation inhibitors , osmotic pressure , and so on , may be further created by using gTME .
	manualset3
139925	2	407503	5	NULL	NULL	0	NULL	enhanced tolerance 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains with enhanced tolerance to other stresses such as heat , fermentation inhibitors , osmotic pressure , and so on , may be further created by using gTME .
	manualset3
139926	3	407503	5	NULL	NULL	0	NULL	stresses 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains with enhanced tolerance to other stresses such as heat , fermentation inhibitors , osmotic pressure , and so on , may be further created by using gTME .
	manualset3
139927	4	407503	5	NULL	NULL	0	NULL	heat 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains with enhanced tolerance to other stresses such as heat , fermentation inhibitors , osmotic pressure , and so on , may be further created by using gTME .
	manualset3
139928	5	407503	5	NULL	NULL	0	NULL	fermentation inhibitors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains with enhanced tolerance to other stresses such as heat , fermentation inhibitors , osmotic pressure , and so on , may be further created by using gTME .
	manualset3
139929	6	407503	5	NULL	NULL	0	NULL	osmotic pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains with enhanced tolerance to other stresses such as heat , fermentation inhibitors , osmotic pressure , and so on , may be further created by using gTME .
	manualset3
139930	7	407503	5	NULL	NULL	0	NULL	 gTME	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains with enhanced tolerance to other stresses such as heat , fermentation inhibitors , osmotic pressure , and so on , may be further created by using gTME .
	manualset3
139931	1	407504	5	NULL	NULL	NULL	NULL	Strains 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Strains with the virulence plasmid could penetrate tissue culture cells irrespective of the original host of the plasmid .
	manualset3
139932	2	407504	5	NULL	NULL	0	NULL	virulence plasmid	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains with the virulence plasmid could penetrate tissue culture cells irrespective of the original host of the plasmid .
	manualset3
139933	3	407504	5	NULL	NULL	0	NULL	tissue culture cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains with the virulence plasmid could penetrate tissue culture cells irrespective of the original host of the plasmid .
	manualset3
139934	4	407504	5	NULL	NULL	NULL	NULL	original host	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Strains with the virulence plasmid could penetrate tissue culture cells irrespective of the original host of the plasmid .
	manualset3
139935	5	407504	5	NULL	NULL	0	NULL	plasmid 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains with the virulence plasmid could penetrate tissue culture cells irrespective of the original host of the plasmid .
	manualset3
139936	1	407505	5	NULL	NULL	0	NULL	Strength training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Strength training following hematopoietic stem cell transplantation .
	manualset3
139937	2	407505	5	NULL	NULL	0	NULL	hematopoietic stem cell transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Strength training following hematopoietic stem cell transplantation .
	manualset3
139938	1	407506	5	NULL	NULL	0	NULL	point mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A point mutation in the putative ATP binding site of the pseudorabies virus US3 protein kinase prevents Bad phosphorylation and cell survival following apoptosis induction .
	manualset3
139939	2	407506	5	NULL	NULL	0	NULL	putative ATP binding site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A point mutation in the putative ATP binding site of the pseudorabies virus US3 protein kinase prevents Bad phosphorylation and cell survival following apoptosis induction .
	manualset3
139940	3	407506	5	NULL	NULL	0	NULL	pseudorabies virus US3 protein kinase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A point mutation in the putative ATP binding site of the pseudorabies virus US3 protein kinase prevents Bad phosphorylation and cell survival following apoptosis induction .
	manualset3
139941	4	407506	5	NULL	NULL	0	NULL	Bad phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A point mutation in the putative ATP binding site of the pseudorabies virus US3 protein kinase prevents Bad phosphorylation and cell survival following apoptosis induction .
	manualset3
139942	5	407506	5	NULL	NULL	0	NULL	cell survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A point mutation in the putative ATP binding site of the pseudorabies virus US3 protein kinase prevents Bad phosphorylation and cell survival following apoptosis induction .
	manualset3
139943	6	407506	5	NULL	NULL	0	NULL	apoptosis induction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A point mutation in the putative ATP binding site of the pseudorabies virus US3 protein kinase prevents Bad phosphorylation and cell survival following apoptosis induction .
	manualset3
139944	1	407507	5	NULL	NULL	0	NULL	Strength training 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Strength training was performed , three times a week for 8 weeks , using a cable pulley simulating the movements in double poling in cross-country skiing , and consisted of three sets of six repetitions at a workload of 85 % of one repetition maximum emphasizing maximal mobilization of force in the concentric movement .
	manualset3
139945	2	407507	5	NULL	NULL	0	NULL	 three times	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Strength training was performed , three times a week for 8 weeks , using a cable pulley simulating the movements in double poling in cross-country skiing , and consisted of three sets of six repetitions at a workload of 85 % of one repetition maximum emphasizing maximal mobilization of force in the concentric movement .
	manualset3
139946	3	407507	5	NULL	NULL	0	NULL	week 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Strength training was performed , three times a week for 8 weeks , using a cable pulley simulating the movements in double poling in cross-country skiing , and consisted of three sets of six repetitions at a workload of 85 % of one repetition maximum emphasizing maximal mobilization of force in the concentric movement .
	manualset3
139947	4	407507	5	NULL	NULL	0	NULL	8 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Strength training was performed , three times a week for 8 weeks , using a cable pulley simulating the movements in double poling in cross-country skiing , and consisted of three sets of six repetitions at a workload of 85 % of one repetition maximum emphasizing maximal mobilization of force in the concentric movement .
	manualset3
139948	5	407507	5	NULL	NULL	0	NULL	cable pulley	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Strength training was performed , three times a week for 8 weeks , using a cable pulley simulating the movements in double poling in cross-country skiing , and consisted of three sets of six repetitions at a workload of 85 % of one repetition maximum emphasizing maximal mobilization of force in the concentric movement .
	manualset3
139949	6	407507	5	NULL	NULL	0	NULL	movements 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Strength training was performed , three times a week for 8 weeks , using a cable pulley simulating the movements in double poling in cross-country skiing , and consisted of three sets of six repetitions at a workload of 85 % of one repetition maximum emphasizing maximal mobilization of force in the concentric movement .
	manualset3
139950	7	407507	5	NULL	NULL	0	NULL	double poling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Strength training was performed , three times a week for 8 weeks , using a cable pulley simulating the movements in double poling in cross-country skiing , and consisted of three sets of six repetitions at a workload of 85 % of one repetition maximum emphasizing maximal mobilization of force in the concentric movement .
	manualset3
139951	8	407507	5	NULL	NULL	0	NULL	cross-country skiing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Strength training was performed , three times a week for 8 weeks , using a cable pulley simulating the movements in double poling in cross-country skiing , and consisted of three sets of six repetitions at a workload of 85 % of one repetition maximum emphasizing maximal mobilization of force in the concentric movement .
	manualset3
139952	9	407507	5	NULL	NULL	0	NULL	three sets	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Strength training was performed , three times a week for 8 weeks , using a cable pulley simulating the movements in double poling in cross-country skiing , and consisted of three sets of six repetitions at a workload of 85 % of one repetition maximum emphasizing maximal mobilization of force in the concentric movement .
	manualset3
139953	10	407507	5	NULL	NULL	0	NULL	six repetitions	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Strength training was performed , three times a week for 8 weeks , using a cable pulley simulating the movements in double poling in cross-country skiing , and consisted of three sets of six repetitions at a workload of 85 % of one repetition maximum emphasizing maximal mobilization of force in the concentric movement .
	manualset3
139954	11	407507	5	NULL	NULL	0	NULL	workload 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Strength training was performed , three times a week for 8 weeks , using a cable pulley simulating the movements in double poling in cross-country skiing , and consisted of three sets of six repetitions at a workload of 85 % of one repetition maximum emphasizing maximal mobilization of force in the concentric movement .
	manualset3
139955	12	407507	5	NULL	NULL	0	NULL	85 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Strength training was performed , three times a week for 8 weeks , using a cable pulley simulating the movements in double poling in cross-country skiing , and consisted of three sets of six repetitions at a workload of 85 % of one repetition maximum emphasizing maximal mobilization of force in the concentric movement .
	manualset3
139956	13	407507	5	NULL	NULL	0	NULL	one repetition	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Strength training was performed , three times a week for 8 weeks , using a cable pulley simulating the movements in double poling in cross-country skiing , and consisted of three sets of six repetitions at a workload of 85 % of one repetition maximum emphasizing maximal mobilization of force in the concentric movement .
	manualset3
139957	14	407507	5	NULL	NULL	0	NULL	maximal mobilization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Strength training was performed , three times a week for 8 weeks , using a cable pulley simulating the movements in double poling in cross-country skiing , and consisted of three sets of six repetitions at a workload of 85 % of one repetition maximum emphasizing maximal mobilization of force in the concentric movement .
	manualset3
139958	15	407507	5	NULL	NULL	0	NULL	force 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Strength training was performed , three times a week for 8 weeks , using a cable pulley simulating the movements in double poling in cross-country skiing , and consisted of three sets of six repetitions at a workload of 85 % of one repetition maximum emphasizing maximal mobilization of force in the concentric movement .
	manualset3
139959	16	407507	5	NULL	NULL	0	NULL	concentric movement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Strength training was performed , three times a week for 8 weeks , using a cable pulley simulating the movements in double poling in cross-country skiing , and consisted of three sets of six repetitions at a workload of 85 % of one repetition maximum emphasizing maximal mobilization of force in the concentric movement .
	manualset3
139960	1	407508	5	NULL	NULL	0	NULL	social capital	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Strengthening social capital in families and communities .
	manualset3
139961	2	407508	5	NULL	NULL	0	NULL	families 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Strengthening social capital in families and communities .
	manualset3
139962	3	407508	5	NULL	NULL	0	NULL	communities 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Strengthening social capital in families and communities .
	manualset3
139963	1	407509	5	NULL	NULL	0	NULL	Streptococcus mutans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Streptococcus mutans : a rare cause of retroperitoneal abscess .
	manualset3
139964	2	407509	5	NULL	NULL	0	NULL	rare cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Streptococcus mutans : a rare cause of retroperitoneal abscess .
	manualset3
139965	3	407509	5	NULL	NULL	0	NULL	retroperitoneal abscess	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Streptococcus mutans : a rare cause of retroperitoneal abscess .
	manualset3
139966	1	407510	5	NULL	NULL	0	NULL	Streptococcus pneumoniae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Streptococcus pneumoniae , one of the main organisms implicated in respiratory tract infections , has developed multiple resistance mechanisms to combat the effects of most commonly used classes of antibiotics , particularly the beta-lactams ( penicillin , aminopenicillins and cephalosporins ) and macrolides .
	manualset3
139967	2	407510	5	NULL	NULL	0	NULL	one 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Streptococcus pneumoniae , one of the main organisms implicated in respiratory tract infections , has developed multiple resistance mechanisms to combat the effects of most commonly used classes of antibiotics , particularly the beta-lactams ( penicillin , aminopenicillins and cephalosporins ) and macrolides .
	manualset3
139968	3	407510	5	NULL	NULL	0	NULL	organisms 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Streptococcus pneumoniae , one of the main organisms implicated in respiratory tract infections , has developed multiple resistance mechanisms to combat the effects of most commonly used classes of antibiotics , particularly the beta-lactams ( penicillin , aminopenicillins and cephalosporins ) and macrolides .
	manualset3
139969	4	407510	5	NULL	NULL	0	NULL	respiratory tract infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Streptococcus pneumoniae , one of the main organisms implicated in respiratory tract infections , has developed multiple resistance mechanisms to combat the effects of most commonly used classes of antibiotics , particularly the beta-lactams ( penicillin , aminopenicillins and cephalosporins ) and macrolides .
	manualset3
139970	5	407510	5	NULL	NULL	0	NULL	multiple resistance mechanisms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Streptococcus pneumoniae , one of the main organisms implicated in respiratory tract infections , has developed multiple resistance mechanisms to combat the effects of most commonly used classes of antibiotics , particularly the beta-lactams ( penicillin , aminopenicillins and cephalosporins ) and macrolides .
	manualset3
139971	6	407510	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Streptococcus pneumoniae , one of the main organisms implicated in respiratory tract infections , has developed multiple resistance mechanisms to combat the effects of most commonly used classes of antibiotics , particularly the beta-lactams ( penicillin , aminopenicillins and cephalosporins ) and macrolides .
	manualset3
139972	7	407510	5	NULL	NULL	0	NULL	classes of antibiotics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Streptococcus pneumoniae , one of the main organisms implicated in respiratory tract infections , has developed multiple resistance mechanisms to combat the effects of most commonly used classes of antibiotics , particularly the beta-lactams ( penicillin , aminopenicillins and cephalosporins ) and macrolides .
	manualset3
139973	8	407510	5	NULL	NULL	0	NULL	beta-lactams	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Streptococcus pneumoniae , one of the main organisms implicated in respiratory tract infections , has developed multiple resistance mechanisms to combat the effects of most commonly used classes of antibiotics , particularly the beta-lactams ( penicillin , aminopenicillins and cephalosporins ) and macrolides .
	manualset3
139974	9	407510	5	NULL	NULL	0	NULL	penicillin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Streptococcus pneumoniae , one of the main organisms implicated in respiratory tract infections , has developed multiple resistance mechanisms to combat the effects of most commonly used classes of antibiotics , particularly the beta-lactams ( penicillin , aminopenicillins and cephalosporins ) and macrolides .
	manualset3
139975	10	407510	5	NULL	NULL	0	NULL	aminopenicillins 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Streptococcus pneumoniae , one of the main organisms implicated in respiratory tract infections , has developed multiple resistance mechanisms to combat the effects of most commonly used classes of antibiotics , particularly the beta-lactams ( penicillin , aminopenicillins and cephalosporins ) and macrolides .
	manualset3
139976	11	407510	5	NULL	NULL	0	NULL	cephalosporins 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Streptococcus pneumoniae , one of the main organisms implicated in respiratory tract infections , has developed multiple resistance mechanisms to combat the effects of most commonly used classes of antibiotics , particularly the beta-lactams ( penicillin , aminopenicillins and cephalosporins ) and macrolides .
	manualset3
139977	12	407510	5	NULL	NULL	0	NULL	macrolides 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Streptococcus pneumoniae , one of the main organisms implicated in respiratory tract infections , has developed multiple resistance mechanisms to combat the effects of most commonly used classes of antibiotics , particularly the beta-lactams ( penicillin , aminopenicillins and cephalosporins ) and macrolides .
	manualset3
139978	1	407511	5	NULL	NULL	0	NULL	Streptococcus pneumoniae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Streptococcus pneumoniae contains many proteins that have not been evaluated as potential protective vaccine antigens .
	manualset3
139979	2	407511	5	NULL	NULL	0	NULL	proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Streptococcus pneumoniae contains many proteins that have not been evaluated as potential protective vaccine antigens .
	manualset3
139980	3	407511	5	NULL	NULL	0	NULL	potential protective vaccine antigens	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Streptococcus pneumoniae contains many proteins that have not been evaluated as potential protective vaccine antigens .
	manualset3
139981	1	407512	5	NULL	NULL	0	NULL	Streptomyces plasmid pSA1 .1	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Streptomyces plasmid pSA1 .1 accumulated single-stranded DNA as replication intermediates in S. lividans ; therefore , this plasmid was considered to replicate by a rolling-circle mechanism .
	manualset3
139982	2	407512	5	NULL	NULL	0	NULL	single-stranded DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Streptomyces plasmid pSA1 .1 accumulated single-stranded DNA as replication intermediates in S. lividans ; therefore , this plasmid was considered to replicate by a rolling-circle mechanism .
	manualset3
139983	3	407512	5	NULL	NULL	0	NULL	replication intermediates 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Streptomyces plasmid pSA1 .1 accumulated single-stranded DNA as replication intermediates in S. lividans ; therefore , this plasmid was considered to replicate by a rolling-circle mechanism .
	manualset3
139984	4	407512	5	NULL	NULL	0	NULL	S. lividans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Streptomyces plasmid pSA1 .1 accumulated single-stranded DNA as replication intermediates in S. lividans ; therefore , this plasmid was considered to replicate by a rolling-circle mechanism .
	manualset3
139985	5	407512	5	NULL	NULL	0	NULL	plasmid 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Streptomyces plasmid pSA1 .1 accumulated single-stranded DNA as replication intermediates in S. lividans ; therefore , this plasmid was considered to replicate by a rolling-circle mechanism .
	manualset3
139986	6	407512	5	NULL	NULL	0	NULL	rolling-circle mechanism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Streptomyces plasmid pSA1 .1 accumulated single-stranded DNA as replication intermediates in S. lividans ; therefore , this plasmid was considered to replicate by a rolling-circle mechanism .
	manualset3
139987	1	407513	5	NULL	NULL	0	NULL	Stress-induced activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stress-induced activation of neuronal activity and corticotropin-releasing factor gene expression in the paraventricular nucleus is modulated by glucocorticoids in rats .
	manualset3
139988	2	407513	5	NULL	NULL	0	NULL	neuronal activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stress-induced activation of neuronal activity and corticotropin-releasing factor gene expression in the paraventricular nucleus is modulated by glucocorticoids in rats .
	manualset3
139989	3	407513	5	NULL	NULL	0	NULL	corticotropin-releasing factor gene expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stress-induced activation of neuronal activity and corticotropin-releasing factor gene expression in the paraventricular nucleus is modulated by glucocorticoids in rats .
	manualset3
139990	4	407513	5	NULL	NULL	0	NULL	paraventricular nucleus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Stress-induced activation of neuronal activity and corticotropin-releasing factor gene expression in the paraventricular nucleus is modulated by glucocorticoids in rats .
	manualset3
139991	5	407513	5	NULL	NULL	0	NULL	glucocorticoids 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Stress-induced activation of neuronal activity and corticotropin-releasing factor gene expression in the paraventricular nucleus is modulated by glucocorticoids in rats .
	manualset3
139992	6	407513	5	NULL	NULL	0	NULL	rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Stress-induced activation of neuronal activity and corticotropin-releasing factor gene expression in the paraventricular nucleus is modulated by glucocorticoids in rats .
	manualset3
139993	1	407514	5	NULL	NULL	0	NULL	polyclonal antiserum	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A polyclonal antiserum was generated against a unique peptide fragment in the rat D4 dopamine ( DA ) receptor .
	manualset3
139994	2	407514	5	NULL	NULL	0	NULL	peptide fragment	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	A polyclonal antiserum was generated against a unique peptide fragment in the rat D4 dopamine ( DA ) receptor .
	manualset3
139995	3	407514	5	NULL	NULL	0	NULL	rat D4 dopamine ( DA ) receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A polyclonal antiserum was generated against a unique peptide fragment in the rat D4 dopamine ( DA ) receptor .
	manualset3
139996	1	407515	5	NULL	NULL	0	NULL	Stress Reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Stress Reduction with Osteopathy Assessed with GDV Electrophotonic Imaging : Effects of Osteopathy Treatment .
	manualset3
139997	2	407515	5	NULL	NULL	0	NULL	Osteopathy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Stress Reduction with Osteopathy Assessed with GDV Electrophotonic Imaging : Effects of Osteopathy Treatment .
	manualset3
139998	3	407515	5	NULL	NULL	0	NULL	 GDV Electrophotonic Imaging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Stress Reduction with Osteopathy Assessed with GDV Electrophotonic Imaging : Effects of Osteopathy Treatment .
	manualset3
139999	4	407515	5	NULL	NULL	0	NULL	Effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Stress Reduction with Osteopathy Assessed with GDV Electrophotonic Imaging : Effects of Osteopathy Treatment .
	manualset3
140000	5	407515	5	NULL	NULL	0	NULL	Osteopathy Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Stress Reduction with Osteopathy Assessed with GDV Electrophotonic Imaging : Effects of Osteopathy Treatment .
	manualset3
140001	1	407516	5	NULL	NULL	0	NULL	Stress 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Stress , distress , and immunity .
	manualset3
140002	2	407516	5	NULL	NULL	0	NULL	distress 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Stress , distress , and immunity .
	manualset3
140003	3	407516	5	NULL	NULL	0	NULL	immunity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stress , distress , and immunity .
	manualset3
140004	1	407517	5	NULL	NULL	0	NULL	Striatal volumes 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Striatal volumes and dyskinetic movements in youth at high-risk for psychosis .
	manualset3
140005	2	407517	5	NULL	NULL	0	NULL	dyskinetic movements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Striatal volumes and dyskinetic movements in youth at high-risk for psychosis .
	manualset3
140006	3	407517	5	NULL	NULL	0	NULL	youth 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Striatal volumes and dyskinetic movements in youth at high-risk for psychosis .
	manualset3
140007	4	407517	5	NULL	NULL	0	NULL	high-risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Striatal volumes and dyskinetic movements in youth at high-risk for psychosis .
	manualset3
140008	5	407517	5	NULL	NULL	0	NULL	psychosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Striatal volumes and dyskinetic movements in youth at high-risk for psychosis .
	manualset3
140009	1	407518	5	NULL	NULL	0	NULL	Strict hygienic practices	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Strict hygienic practices or the implementation of decontamination technologies is recommended .
	manualset3
140010	2	407518	5	NULL	NULL	0	NULL	implementation of decontamination technologies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Strict hygienic practices or the implementation of decontamination technologies is recommended .
	manualset3
140011	1	407519	5	NULL	NULL	NULL	NULL	bactericidal activity 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Striking bactericidal activity against five strains was achieved by the combination , whereas neither drug alone in low dosage was capable of bactericidal action .
	manualset3
140012	2	407519	5	NULL	NULL	0	NULL	five 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Striking bactericidal activity against five strains was achieved by the combination , whereas neither drug alone in low dosage was capable of bactericidal action .
	manualset3
140013	3	407519	5	NULL	NULL	0	NULL	strains 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Striking bactericidal activity against five strains was achieved by the combination , whereas neither drug alone in low dosage was capable of bactericidal action .
	manualset3
140014	4	407519	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Striking bactericidal activity against five strains was achieved by the combination , whereas neither drug alone in low dosage was capable of bactericidal action .
	manualset3
140015	5	407519	5	NULL	NULL	0	NULL	drug 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Striking bactericidal activity against five strains was achieved by the combination , whereas neither drug alone in low dosage was capable of bactericidal action .
	manualset3
140016	6	407519	5	NULL	NULL	0	NULL	low dosage 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Striking bactericidal activity against five strains was achieved by the combination , whereas neither drug alone in low dosage was capable of bactericidal action .
	manualset3
140017	7	407519	5	NULL	NULL	0	NULL	bactericidal action	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Striking bactericidal activity against five strains was achieved by the combination , whereas neither drug alone in low dosage was capable of bactericidal action .
	manualset3
140018	1	407520	5	NULL	NULL	0	NULL	steady-state messenger RNA ( mRNA ) levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Strikingly , steady-state messenger RNA ( mRNA ) levels of VEGF-A and - B and the major bone resorption stimulators PTHrP and M-CSF by tumor cells were elevated significantly in bone versus soft tissues ( p & lt ; or = 0.05 , p & lt ; or = 0.0001 , p & lt ; or = 0.001 , and p & lt ; or = 0.05 , respectively ) , indicating tissue-specific expression of these tumor progression factors .
	manualset3
140019	2	407520	5	NULL	NULL	0	NULL	VEGF-A	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Strikingly , steady-state messenger RNA ( mRNA ) levels of VEGF-A and - B and the major bone resorption stimulators PTHrP and M-CSF by tumor cells were elevated significantly in bone versus soft tissues ( p & lt ; or = 0.05 , p & lt ; or = 0.0001 , p & lt ; or = 0.001 , and p & lt ; or = 0.05 , respectively ) , indicating tissue-specific expression of these tumor progression factors .
	manualset3
140020	3	407520	5	NULL	NULL	0	NULL	VEGF-B	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Strikingly , steady-state messenger RNA ( mRNA ) levels of VEGF-A and - B and the major bone resorption stimulators PTHrP and M-CSF by tumor cells were elevated significantly in bone versus soft tissues ( p & lt ; or = 0.05 , p & lt ; or = 0.0001 , p & lt ; or = 0.001 , and p & lt ; or = 0.05 , respectively ) , indicating tissue-specific expression of these tumor progression factors .
	manualset3
140021	4	407520	5	NULL	NULL	0	NULL	 bone resorption stimulator PTHrP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Strikingly , steady-state messenger RNA ( mRNA ) levels of VEGF-A and - B and the major bone resorption stimulators PTHrP and M-CSF by tumor cells were elevated significantly in bone versus soft tissues ( p & lt ; or = 0.05 , p & lt ; or = 0.0001 , p & lt ; or = 0.001 , and p & lt ; or = 0.05 , respectively ) , indicating tissue-specific expression of these tumor progression factors .
	manualset3
140022	5	407520	5	NULL	NULL	0	NULL	 bone resorption stimulator M-CSF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Strikingly , steady-state messenger RNA ( mRNA ) levels of VEGF-A and - B and the major bone resorption stimulators PTHrP and M-CSF by tumor cells were elevated significantly in bone versus soft tissues ( p & lt ; or = 0.05 , p & lt ; or = 0.0001 , p & lt ; or = 0.001 , and p & lt ; or = 0.05 , respectively ) , indicating tissue-specific expression of these tumor progression factors .
	manualset3
140023	6	407520	5	NULL	NULL	0	NULL	tumor cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Strikingly , steady-state messenger RNA ( mRNA ) levels of VEGF-A and - B and the major bone resorption stimulators PTHrP and M-CSF by tumor cells were elevated significantly in bone versus soft tissues ( p & lt ; or = 0.05 , p & lt ; or = 0.0001 , p & lt ; or = 0.001 , and p & lt ; or = 0.05 , respectively ) , indicating tissue-specific expression of these tumor progression factors .
	manualset3
140024	7	407520	5	NULL	NULL	0	NULL	bone 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Strikingly , steady-state messenger RNA ( mRNA ) levels of VEGF-A and - B and the major bone resorption stimulators PTHrP and M-CSF by tumor cells were elevated significantly in bone versus soft tissues ( p & lt ; or = 0.05 , p & lt ; or = 0.0001 , p & lt ; or = 0.001 , and p & lt ; or = 0.05 , respectively ) , indicating tissue-specific expression of these tumor progression factors .
	manualset3
140025	8	407520	5	NULL	NULL	0	NULL	soft tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Strikingly , steady-state messenger RNA ( mRNA ) levels of VEGF-A and - B and the major bone resorption stimulators PTHrP and M-CSF by tumor cells were elevated significantly in bone versus soft tissues ( p & lt ; or = 0.05 , p & lt ; or = 0.0001 , p & lt ; or = 0.001 , and p & lt ; or = 0.05 , respectively ) , indicating tissue-specific expression of these tumor progression factors .
	manualset3
140026	9	407520	5	NULL	NULL	0	NULL	p & lt ; or = 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Strikingly , steady-state messenger RNA ( mRNA ) levels of VEGF-A and - B and the major bone resorption stimulators PTHrP and M-CSF by tumor cells were elevated significantly in bone versus soft tissues ( p & lt ; or = 0.05 , p & lt ; or = 0.0001 , p & lt ; or = 0.001 , and p & lt ; or = 0.05 , respectively ) , indicating tissue-specific expression of these tumor progression factors .
	manualset3
140027	10	407520	5	NULL	NULL	0	NULL	p & lt ; or = 0.0001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Strikingly , steady-state messenger RNA ( mRNA ) levels of VEGF-A and - B and the major bone resorption stimulators PTHrP and M-CSF by tumor cells were elevated significantly in bone versus soft tissues ( p & lt ; or = 0.05 , p & lt ; or = 0.0001 , p & lt ; or = 0.001 , and p & lt ; or = 0.05 , respectively ) , indicating tissue-specific expression of these tumor progression factors .
	manualset3
140028	11	407520	5	NULL	NULL	0	NULL	p & lt ; or = 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Strikingly , steady-state messenger RNA ( mRNA ) levels of VEGF-A and - B and the major bone resorption stimulators PTHrP and M-CSF by tumor cells were elevated significantly in bone versus soft tissues ( p & lt ; or = 0.05 , p & lt ; or = 0.0001 , p & lt ; or = 0.001 , and p & lt ; or = 0.05 , respectively ) , indicating tissue-specific expression of these tumor progression factors .
	manualset3
140029	12	407520	5	NULL	NULL	0	NULL	p & lt ; or = 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Strikingly , steady-state messenger RNA ( mRNA ) levels of VEGF-A and - B and the major bone resorption stimulators PTHrP and M-CSF by tumor cells were elevated significantly in bone versus soft tissues ( p & lt ; or = 0.05 , p & lt ; or = 0.0001 , p & lt ; or = 0.001 , and p & lt ; or = 0.05 , respectively ) , indicating tissue-specific expression of these tumor progression factors .
	manualset3
140030	13	407520	5	NULL	NULL	0	NULL	tissue-specific expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Strikingly , steady-state messenger RNA ( mRNA ) levels of VEGF-A and - B and the major bone resorption stimulators PTHrP and M-CSF by tumor cells were elevated significantly in bone versus soft tissues ( p & lt ; or = 0.05 , p & lt ; or = 0.0001 , p & lt ; or = 0.001 , and p & lt ; or = 0.05 , respectively ) , indicating tissue-specific expression of these tumor progression factors .
	manualset3
140031	14	407520	5	NULL	NULL	0	NULL	tumor progression factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Strikingly , steady-state messenger RNA ( mRNA ) levels of VEGF-A and - B and the major bone resorption stimulators PTHrP and M-CSF by tumor cells were elevated significantly in bone versus soft tissues ( p & lt ; or = 0.05 , p & lt ; or = 0.0001 , p & lt ; or = 0.001 , and p & lt ; or = 0.05 , respectively ) , indicating tissue-specific expression of these tumor progression factors .
	manualset3
140032	1	407521	5	NULL	NULL	0	NULL	polymorphism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A polymorphism of the human Brain Derived Neurotrophic Factor ( BDNF ) gene that produces a valine-to-methionine substitution at codon 66 ( Val66Met ) is linked to adult anxiety and mood disorders , possibly through effects on brain circuitry function .
	manualset3
140033	2	407521	5	NULL	NULL	0	NULL	human Brain Derived Neurotrophic Factor ( BDNF ) gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A polymorphism of the human Brain Derived Neurotrophic Factor ( BDNF ) gene that produces a valine-to-methionine substitution at codon 66 ( Val66Met ) is linked to adult anxiety and mood disorders , possibly through effects on brain circuitry function .
	manualset3
140034	3	407521	5	NULL	NULL	NULL	NULL	 valine-to-methionine substitution at codon 66 ( Val66Met ) 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A polymorphism of the human Brain Derived Neurotrophic Factor ( BDNF ) gene that produces a valine-to-methionine substitution at codon 66 ( Val66Met ) is linked to adult anxiety and mood disorders , possibly through effects on brain circuitry function .
	manualset3
140035	4	407521	5	NULL	NULL	0	NULL	adult anxiety 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A polymorphism of the human Brain Derived Neurotrophic Factor ( BDNF ) gene that produces a valine-to-methionine substitution at codon 66 ( Val66Met ) is linked to adult anxiety and mood disorders , possibly through effects on brain circuitry function .
	manualset3
140036	5	407521	5	NULL	NULL	0	NULL	mood disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A polymorphism of the human Brain Derived Neurotrophic Factor ( BDNF ) gene that produces a valine-to-methionine substitution at codon 66 ( Val66Met ) is linked to adult anxiety and mood disorders , possibly through effects on brain circuitry function .
	manualset3
140037	6	407521	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A polymorphism of the human Brain Derived Neurotrophic Factor ( BDNF ) gene that produces a valine-to-methionine substitution at codon 66 ( Val66Met ) is linked to adult anxiety and mood disorders , possibly through effects on brain circuitry function .
	manualset3
140038	7	407521	5	NULL	NULL	0	NULL	brain circuitry function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A polymorphism of the human Brain Derived Neurotrophic Factor ( BDNF ) gene that produces a valine-to-methionine substitution at codon 66 ( Val66Met ) is linked to adult anxiety and mood disorders , possibly through effects on brain circuitry function .
	manualset3
140039	1	407522	5	NULL	NULL	0	NULL	Stroke 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Stroke produces a loss of physiological brain maps in adjacent peri-infarct cortex and then a remapping of motor and sensory functions in this region .
	manualset3
140040	2	407522	5	NULL	NULL	NULL	NULL	loss of physiological brain maps	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Stroke produces a loss of physiological brain maps in adjacent peri-infarct cortex and then a remapping of motor and sensory functions in this region .
	manualset3
140041	3	407522	5	NULL	NULL	0	NULL	peri-infarct cortex 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Stroke produces a loss of physiological brain maps in adjacent peri-infarct cortex and then a remapping of motor and sensory functions in this region .
	manualset3
140042	4	407522	5	NULL	NULL	0	NULL	motor functions 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stroke produces a loss of physiological brain maps in adjacent peri-infarct cortex and then a remapping of motor and sensory functions in this region .
	manualset3
140043	5	407522	5	NULL	NULL	0	NULL	sensory functions 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stroke produces a loss of physiological brain maps in adjacent peri-infarct cortex and then a remapping of motor and sensory functions in this region .
	manualset3
140044	6	407522	5	NULL	NULL	0	NULL	region 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Stroke produces a loss of physiological brain maps in adjacent peri-infarct cortex and then a remapping of motor and sensory functions in this region .
	manualset3
140045	1	407523	5	NULL	NULL	0	NULL	Stroma-derived matrix metalloproteinase ( MMP ) -2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Stroma-derived matrix metalloproteinase ( MMP ) -2 promotes membrane type 1-MMP-dependent tumor growth in mice .
	manualset3
140046	2	407523	5	NULL	NULL	0	NULL	membrane type 1-MMP-dependent tumor growth 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stroma-derived matrix metalloproteinase ( MMP ) -2 promotes membrane type 1-MMP-dependent tumor growth in mice .
	manualset3
140047	3	407523	5	NULL	NULL	0	NULL	mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Stroma-derived matrix metalloproteinase ( MMP ) -2 promotes membrane type 1-MMP-dependent tumor growth in mice .
	manualset3
140048	1	407524	5	NULL	NULL	0	NULL	correlations 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Strong correlations were also found between the pEC20 values for potentiation of the twitch response and the pKi values for bovine cardiac M2 muscarinic receptors and between the pIC50 values for inhibition of the twitch response and the pA2 values for M3 muscarinic receptors as determined on non-stimulated methacholine-contracted tracheal smooth muscle preparations .
	manualset3
140049	2	407524	5	NULL	NULL	0	NULL	pEC20 values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Strong correlations were also found between the pEC20 values for potentiation of the twitch response and the pKi values for bovine cardiac M2 muscarinic receptors and between the pIC50 values for inhibition of the twitch response and the pA2 values for M3 muscarinic receptors as determined on non-stimulated methacholine-contracted tracheal smooth muscle preparations .
	manualset3
140050	3	407524	5	NULL	NULL	0	NULL	potentiation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Strong correlations were also found between the pEC20 values for potentiation of the twitch response and the pKi values for bovine cardiac M2 muscarinic receptors and between the pIC50 values for inhibition of the twitch response and the pA2 values for M3 muscarinic receptors as determined on non-stimulated methacholine-contracted tracheal smooth muscle preparations .
	manualset3
140051	4	407524	5	NULL	NULL	NULL	NULL	twitch response	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Strong correlations were also found between the pEC20 values for potentiation of the twitch response and the pKi values for bovine cardiac M2 muscarinic receptors and between the pIC50 values for inhibition of the twitch response and the pA2 values for M3 muscarinic receptors as determined on non-stimulated methacholine-contracted tracheal smooth muscle preparations .
	manualset3
140052	5	407524	5	NULL	NULL	0	NULL	pKi values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Strong correlations were also found between the pEC20 values for potentiation of the twitch response and the pKi values for bovine cardiac M2 muscarinic receptors and between the pIC50 values for inhibition of the twitch response and the pA2 values for M3 muscarinic receptors as determined on non-stimulated methacholine-contracted tracheal smooth muscle preparations .
	manualset3
140053	6	407524	5	NULL	NULL	0	NULL	bovine cardiac M2 muscarinic receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Strong correlations were also found between the pEC20 values for potentiation of the twitch response and the pKi values for bovine cardiac M2 muscarinic receptors and between the pIC50 values for inhibition of the twitch response and the pA2 values for M3 muscarinic receptors as determined on non-stimulated methacholine-contracted tracheal smooth muscle preparations .
	manualset3
140054	7	407524	5	NULL	NULL	0	NULL	pIC50 values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Strong correlations were also found between the pEC20 values for potentiation of the twitch response and the pKi values for bovine cardiac M2 muscarinic receptors and between the pIC50 values for inhibition of the twitch response and the pA2 values for M3 muscarinic receptors as determined on non-stimulated methacholine-contracted tracheal smooth muscle preparations .
	manualset3
140055	8	407524	5	NULL	NULL	0	NULL	inhibition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Strong correlations were also found between the pEC20 values for potentiation of the twitch response and the pKi values for bovine cardiac M2 muscarinic receptors and between the pIC50 values for inhibition of the twitch response and the pA2 values for M3 muscarinic receptors as determined on non-stimulated methacholine-contracted tracheal smooth muscle preparations .
	manualset3
140056	9	407524	5	NULL	NULL	NULL	NULL	twitch response	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Strong correlations were also found between the pEC20 values for potentiation of the twitch response and the pKi values for bovine cardiac M2 muscarinic receptors and between the pIC50 values for inhibition of the twitch response and the pA2 values for M3 muscarinic receptors as determined on non-stimulated methacholine-contracted tracheal smooth muscle preparations .
	manualset3
140057	10	407524	5	NULL	NULL	0	NULL	pA2 values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Strong correlations were also found between the pEC20 values for potentiation of the twitch response and the pKi values for bovine cardiac M2 muscarinic receptors and between the pIC50 values for inhibition of the twitch response and the pA2 values for M3 muscarinic receptors as determined on non-stimulated methacholine-contracted tracheal smooth muscle preparations .
	manualset3
140058	11	407524	5	NULL	NULL	0	NULL	M3 muscarinic receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Strong correlations were also found between the pEC20 values for potentiation of the twitch response and the pKi values for bovine cardiac M2 muscarinic receptors and between the pIC50 values for inhibition of the twitch response and the pA2 values for M3 muscarinic receptors as determined on non-stimulated methacholine-contracted tracheal smooth muscle preparations .
	manualset3
140059	12	407524	5	NULL	NULL	0	NULL	non-stimulated methacholine-contracted tracheal smooth muscle preparations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Strong correlations were also found between the pEC20 values for potentiation of the twitch response and the pKi values for bovine cardiac M2 muscarinic receptors and between the pIC50 values for inhibition of the twitch response and the pA2 values for M3 muscarinic receptors as determined on non-stimulated methacholine-contracted tracheal smooth muscle preparations .
	manualset3
140060	1	407525	5	NULL	NULL	0	NULL	Strong sequence conservation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Strong sequence conservation of African swine fever virus p72 protein provides the molecular basis for its antigenic stability .
	manualset3
140061	2	407525	5	NULL	NULL	0	NULL	African swine fever virus p72 protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Strong sequence conservation of African swine fever virus p72 protein provides the molecular basis for its antigenic stability .
	manualset3
140062	3	407525	5	NULL	NULL	0	NULL	molecular basis	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Strong sequence conservation of African swine fever virus p72 protein provides the molecular basis for its antigenic stability .
	manualset3
140063	4	407525	5	NULL	NULL	0	NULL	antigenic stability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Strong sequence conservation of African swine fever virus p72 protein provides the molecular basis for its antigenic stability .
	manualset3
140064	1	407526	5	NULL	NULL	0	NULL	ultraviolet luminescence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Strong ultraviolet luminescence of ZnO thin films with nanowall-network structures .
	manualset3
140065	2	407526	5	NULL	NULL	0	NULL	ZnO thin films 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Strong ultraviolet luminescence of ZnO thin films with nanowall-network structures .
	manualset3
140066	3	407526	5	NULL	NULL	0	NULL	nanowall-network structures	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Strong ultraviolet luminescence of ZnO thin films with nanowall-network structures .
	manualset3
140067	1	407527	5	NULL	NULL	0	NULL	excision 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Strongest excision ( & gt ; 50 % ) was observed when the loxP cassette was cloned into vector pPZP112 and Cre into pISV2678 .
	manualset3
140068	2	407527	5	NULL	NULL	0	NULL	& gt ; 50 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Strongest excision ( & gt ; 50 % ) was observed when the loxP cassette was cloned into vector pPZP112 and Cre into pISV2678 .
	manualset3
140069	3	407527	5	NULL	NULL	0	NULL	 loxP cassette	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Strongest excision ( & gt ; 50 % ) was observed when the loxP cassette was cloned into vector pPZP112 and Cre into pISV2678 .
	manualset3
140070	4	407527	5	NULL	NULL	0	NULL	vector pPZP112	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Strongest excision ( & gt ; 50 % ) was observed when the loxP cassette was cloned into vector pPZP112 and Cre into pISV2678 .
	manualset3
140071	5	407527	5	NULL	NULL	0	NULL	Cre	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Strongest excision ( & gt ; 50 % ) was observed when the loxP cassette was cloned into vector pPZP112 and Cre into pISV2678 .
	manualset3
140072	6	407527	5	NULL	NULL	0	NULL	pISV2678 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Strongest excision ( & gt ; 50 % ) was observed when the loxP cassette was cloned into vector pPZP112 and Cre into pISV2678 .
	manualset3
140073	1	407528	5	NULL	NULL	0	NULL	population descriptive analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A population descriptive analysis is done with medians and description of the etiology .
	manualset3
140074	2	407528	5	NULL	NULL	0	NULL	medians 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A population descriptive analysis is done with medians and description of the etiology .
	manualset3
140075	3	407528	5	NULL	NULL	0	NULL	description 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A population descriptive analysis is done with medians and description of the etiology .
	manualset3
140076	4	407528	5	NULL	NULL	NULL	NULL	etiology 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A population descriptive analysis is done with medians and description of the etiology .
	manualset3
140080	1	407529	5	NULL	NULL	0	NULL	Structural evidence 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural , vibrational , and NMR spectroscopic evidence is given for a successive weakening of the pi back-bonding effect of the W-P bond in the order ( W ( CO ) ( 5 ) PH ( R ( f ) ) ( 2 ) ) , ( Hg ( ( mu-P ( R ( f ) ) ( 2 ) ) W ( CO ) ( 5 ) ) ( 2 ) ) , and ( W ( P ( R ( f ) ) ( 2 ) ) ( CO ) ( 5 ) ) ( - ) with R ( f ) = C ( 6 ) F ( 5 ) and CF ( 3 ) .
	manualset3
140081	2	407529	5	NULL	NULL	0	NULL	vibrational evidence 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural , vibrational , and NMR spectroscopic evidence is given for a successive weakening of the pi back-bonding effect of the W-P bond in the order ( W ( CO ) ( 5 ) PH ( R ( f ) ) ( 2 ) ) , ( Hg ( ( mu-P ( R ( f ) ) ( 2 ) ) W ( CO ) ( 5 ) ) ( 2 ) ) , and ( W ( P ( R ( f ) ) ( 2 ) ) ( CO ) ( 5 ) ) ( - ) with R ( f ) = C ( 6 ) F ( 5 ) and CF ( 3 ) .
	manualset3
140082	3	407529	5	NULL	NULL	0	NULL	NMR spectroscopic evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural , vibrational , and NMR spectroscopic evidence is given for a successive weakening of the pi back-bonding effect of the W-P bond in the order ( W ( CO ) ( 5 ) PH ( R ( f ) ) ( 2 ) ) , ( Hg ( ( mu-P ( R ( f ) ) ( 2 ) ) W ( CO ) ( 5 ) ) ( 2 ) ) , and ( W ( P ( R ( f ) ) ( 2 ) ) ( CO ) ( 5 ) ) ( - ) with R ( f ) = C ( 6 ) F ( 5 ) and CF ( 3 ) .
	manualset3
140083	4	407529	5	NULL	NULL	0	NULL	pi back-bonding effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural , vibrational , and NMR spectroscopic evidence is given for a successive weakening of the pi back-bonding effect of the W-P bond in the order ( W ( CO ) ( 5 ) PH ( R ( f ) ) ( 2 ) ) , ( Hg ( ( mu-P ( R ( f ) ) ( 2 ) ) W ( CO ) ( 5 ) ) ( 2 ) ) , and ( W ( P ( R ( f ) ) ( 2 ) ) ( CO ) ( 5 ) ) ( - ) with R ( f ) = C ( 6 ) F ( 5 ) and CF ( 3 ) .
	manualset3
140084	5	407529	5	NULL	NULL	0	NULL	W-P bond	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural , vibrational , and NMR spectroscopic evidence is given for a successive weakening of the pi back-bonding effect of the W-P bond in the order ( W ( CO ) ( 5 ) PH ( R ( f ) ) ( 2 ) ) , ( Hg ( ( mu-P ( R ( f ) ) ( 2 ) ) W ( CO ) ( 5 ) ) ( 2 ) ) , and ( W ( P ( R ( f ) ) ( 2 ) ) ( CO ) ( 5 ) ) ( - ) with R ( f ) = C ( 6 ) F ( 5 ) and CF ( 3 ) .
	manualset3
140085	6	407529	5	NULL	NULL	0	NULL	( W ( CO ) ( 5 ) PH ( R ( f ) ) ( 2 ) )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural , vibrational , and NMR spectroscopic evidence is given for a successive weakening of the pi back-bonding effect of the W-P bond in the order ( W ( CO ) ( 5 ) PH ( R ( f ) ) ( 2 ) ) , ( Hg ( ( mu-P ( R ( f ) ) ( 2 ) ) W ( CO ) ( 5 ) ) ( 2 ) ) , and ( W ( P ( R ( f ) ) ( 2 ) ) ( CO ) ( 5 ) ) ( - ) with R ( f ) = C ( 6 ) F ( 5 ) and CF ( 3 ) .
	manualset3
140086	7	407529	5	NULL	NULL	0	NULL	( Hg ( ( mu-P ( R ( f ) ) ( 2 ) ) W ( CO ) ( 5 ) ) ( 2 ) )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural , vibrational , and NMR spectroscopic evidence is given for a successive weakening of the pi back-bonding effect of the W-P bond in the order ( W ( CO ) ( 5 ) PH ( R ( f ) ) ( 2 ) ) , ( Hg ( ( mu-P ( R ( f ) ) ( 2 ) ) W ( CO ) ( 5 ) ) ( 2 ) ) , and ( W ( P ( R ( f ) ) ( 2 ) ) ( CO ) ( 5 ) ) ( - ) with R ( f ) = C ( 6 ) F ( 5 ) and CF ( 3 ) .
	manualset3
140087	8	407529	5	NULL	NULL	0	NULL	( W ( P ( R ( f ) ) ( 2 ) ) ( CO ) ( 5 ) ) ( - ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural , vibrational , and NMR spectroscopic evidence is given for a successive weakening of the pi back-bonding effect of the W-P bond in the order ( W ( CO ) ( 5 ) PH ( R ( f ) ) ( 2 ) ) , ( Hg ( ( mu-P ( R ( f ) ) ( 2 ) ) W ( CO ) ( 5 ) ) ( 2 ) ) , and ( W ( P ( R ( f ) ) ( 2 ) ) ( CO ) ( 5 ) ) ( - ) with R ( f ) = C ( 6 ) F ( 5 ) and CF ( 3 ) .
	manualset3
140088	9	407529	5	NULL	NULL	0	NULL	R ( f ) = C ( 6 ) F ( 5 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural , vibrational , and NMR spectroscopic evidence is given for a successive weakening of the pi back-bonding effect of the W-P bond in the order ( W ( CO ) ( 5 ) PH ( R ( f ) ) ( 2 ) ) , ( Hg ( ( mu-P ( R ( f ) ) ( 2 ) ) W ( CO ) ( 5 ) ) ( 2 ) ) , and ( W ( P ( R ( f ) ) ( 2 ) ) ( CO ) ( 5 ) ) ( - ) with R ( f ) = C ( 6 ) F ( 5 ) and CF ( 3 ) .
	manualset3
140089	10	407529	5	NULL	NULL	0	NULL	CF ( 3 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural , vibrational , and NMR spectroscopic evidence is given for a successive weakening of the pi back-bonding effect of the W-P bond in the order ( W ( CO ) ( 5 ) PH ( R ( f ) ) ( 2 ) ) , ( Hg ( ( mu-P ( R ( f ) ) ( 2 ) ) W ( CO ) ( 5 ) ) ( 2 ) ) , and ( W ( P ( R ( f ) ) ( 2 ) ) ( CO ) ( 5 ) ) ( - ) with R ( f ) = C ( 6 ) F ( 5 ) and CF ( 3 ) .
	manualset3
140077	1	407530	5	NULL	NULL	0	NULL	Structural properties 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural and biologic properties of a human aspartic acid-126 interleukin-2 analog .
	manualset3
140078	2	407530	5	NULL	NULL	0	NULL	biologic properties 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural and biologic properties of a human aspartic acid-126 interleukin-2 analog .
	manualset3
140079	3	407530	5	NULL	NULL	0	NULL	human aspartic acid-126 interleukin-2 analog	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural and biologic properties of a human aspartic acid-126 interleukin-2 analog .
	manualset3
136521	1	407531	13	NULL	NULL	0	NULL	Structural characteristics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural characteristics of goat ( Capra hircus ) parotid salivary glands .
	manualset3
136523	2	407531	13	NULL	NULL	NULL	NULL	goat ( Capra hircus ) 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Structural characteristics of goat ( Capra hircus ) parotid salivary glands .
	manualset3
136528	3	407531	13	NULL	NULL	0	NULL	parotid salivary glands	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural characteristics of goat ( Capra hircus ) parotid salivary glands .
	manualset3
136531	1	407532	13	NULL	NULL	0	NULL	Structural genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural genes for DAHP synthase isoenzymes in Neurospora crassa .
	manualset3
136533	2	407532	13	NULL	NULL	0	NULL	DAHP synthase isoenzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural genes for DAHP synthase isoenzymes in Neurospora crassa .
	manualset3
136534	3	407532	13	NULL	NULL	0	NULL	Neurospora crassa 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural genes for DAHP synthase isoenzymes in Neurospora crassa .
	manualset3
136554	1	407533	13	NULL	NULL	0	NULL	Structural insights	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural insights into the function of the Rab GDI superfamily .
	manualset3
136555	2	407533	13	NULL	NULL	0	NULL	function 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural insights into the function of the Rab GDI superfamily .
	manualset3
136556	3	407533	13	NULL	NULL	0	NULL	Rab GDI superfamily	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural insights into the function of the Rab GDI superfamily .
	manualset3
136557	1	407534	13	NULL	NULL	0	NULL	Structural parameters	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural parameters , thermodynamic properties of oligomerization reaction , band gaps , and dipole moments of the 18 lowest-energy structures of the studied heptamers in each series are compared to their corresponding binary parents , that is , ( ( HM ) ( 7 ) ( NH ) ( 7 ) ) and ( ( HGa ) ( 7 ) ( YH ) ( 7 ) ) .
	manualset3
136558	2	407534	13	NULL	NULL	0	NULL	thermodynamic properties	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural parameters , thermodynamic properties of oligomerization reaction , band gaps , and dipole moments of the 18 lowest-energy structures of the studied heptamers in each series are compared to their corresponding binary parents , that is , ( ( HM ) ( 7 ) ( NH ) ( 7 ) ) and ( ( HGa ) ( 7 ) ( YH ) ( 7 ) ) .
	manualset3
136559	3	407534	13	NULL	NULL	0	NULL	oligomerization reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural parameters , thermodynamic properties of oligomerization reaction , band gaps , and dipole moments of the 18 lowest-energy structures of the studied heptamers in each series are compared to their corresponding binary parents , that is , ( ( HM ) ( 7 ) ( NH ) ( 7 ) ) and ( ( HGa ) ( 7 ) ( YH ) ( 7 ) ) .
	manualset3
136560	4	407534	13	NULL	NULL	0	NULL	band gaps	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural parameters , thermodynamic properties of oligomerization reaction , band gaps , and dipole moments of the 18 lowest-energy structures of the studied heptamers in each series are compared to their corresponding binary parents , that is , ( ( HM ) ( 7 ) ( NH ) ( 7 ) ) and ( ( HGa ) ( 7 ) ( YH ) ( 7 ) ) .
	manualset3
136561	5	407534	13	NULL	NULL	0	NULL	dipole moments	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural parameters , thermodynamic properties of oligomerization reaction , band gaps , and dipole moments of the 18 lowest-energy structures of the studied heptamers in each series are compared to their corresponding binary parents , that is , ( ( HM ) ( 7 ) ( NH ) ( 7 ) ) and ( ( HGa ) ( 7 ) ( YH ) ( 7 ) ) .
	manualset3
136562	6	407534	13	NULL	NULL	0	NULL	18 lowest-energy structures	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural parameters , thermodynamic properties of oligomerization reaction , band gaps , and dipole moments of the 18 lowest-energy structures of the studied heptamers in each series are compared to their corresponding binary parents , that is , ( ( HM ) ( 7 ) ( NH ) ( 7 ) ) and ( ( HGa ) ( 7 ) ( YH ) ( 7 ) ) .
	manualset3
136563	7	407534	13	NULL	NULL	0	NULL	heptamers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural parameters , thermodynamic properties of oligomerization reaction , band gaps , and dipole moments of the 18 lowest-energy structures of the studied heptamers in each series are compared to their corresponding binary parents , that is , ( ( HM ) ( 7 ) ( NH ) ( 7 ) ) and ( ( HGa ) ( 7 ) ( YH ) ( 7 ) ) .
	manualset3
136564	8	407534	13	NULL	NULL	0	NULL	binary parents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural parameters , thermodynamic properties of oligomerization reaction , band gaps , and dipole moments of the 18 lowest-energy structures of the studied heptamers in each series are compared to their corresponding binary parents , that is , ( ( HM ) ( 7 ) ( NH ) ( 7 ) ) and ( ( HGa ) ( 7 ) ( YH ) ( 7 ) ) .
	manualset3
136565	9	407534	13	NULL	NULL	0	NULL	( ( HM ) ( 7 ) ( NH ) ( 7 ) ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural parameters , thermodynamic properties of oligomerization reaction , band gaps , and dipole moments of the 18 lowest-energy structures of the studied heptamers in each series are compared to their corresponding binary parents , that is , ( ( HM ) ( 7 ) ( NH ) ( 7 ) ) and ( ( HGa ) ( 7 ) ( YH ) ( 7 ) ) .
	manualset3
136566	10	407534	13	NULL	NULL	0	NULL	( ( HGa ) ( 7 ) ( YH ) ( 7 ) )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural parameters , thermodynamic properties of oligomerization reaction , band gaps , and dipole moments of the 18 lowest-energy structures of the studied heptamers in each series are compared to their corresponding binary parents , that is , ( ( HM ) ( 7 ) ( NH ) ( 7 ) ) and ( ( HGa ) ( 7 ) ( YH ) ( 7 ) ) .
	manualset3
136567	11	407534	13	NULL	NULL	0	NULL	series	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural parameters , thermodynamic properties of oligomerization reaction , band gaps , and dipole moments of the 18 lowest-energy structures of the studied heptamers in each series are compared to their corresponding binary parents , that is , ( ( HM ) ( 7 ) ( NH ) ( 7 ) ) and ( ( HGa ) ( 7 ) ( YH ) ( 7 ) ) .
	manualset3
136568	1	407535	13	NULL	NULL	0	NULL	Structural similarities	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural similarities between thiamin-binding protein and thiaminase-I suggest a common ancestor .
	manualset3
136569	2	407535	13	NULL	NULL	0	NULL	thiamin-binding protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural similarities between thiamin-binding protein and thiaminase-I suggest a common ancestor .
	manualset3
136570	3	407535	13	NULL	NULL	0	NULL	thiaminase-I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural similarities between thiamin-binding protein and thiaminase-I suggest a common ancestor .
	manualset3
136571	4	407535	13	NULL	NULL	0	NULL	 common ancestor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural similarities between thiamin-binding protein and thiaminase-I suggest a common ancestor .
	manualset3
136572	1	407536	13	NULL	NULL	0	NULL	population	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A population of plasma cells was also identified in the peripheral blood of patient Ei that showed strong intracellular staining with the idiotypic antiserum and was the apparent source of the specific serum immunoglobulin .
	manualset3
136573	2	407536	13	NULL	NULL	0	NULL	plasma cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A population of plasma cells was also identified in the peripheral blood of patient Ei that showed strong intracellular staining with the idiotypic antiserum and was the apparent source of the specific serum immunoglobulin .
	manualset3
136574	3	407536	13	NULL	NULL	0	NULL	peripheral blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	A population of plasma cells was also identified in the peripheral blood of patient Ei that showed strong intracellular staining with the idiotypic antiserum and was the apparent source of the specific serum immunoglobulin .
	manualset3
136575	4	407536	13	NULL	NULL	0	NULL	patient Ei 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A population of plasma cells was also identified in the peripheral blood of patient Ei that showed strong intracellular staining with the idiotypic antiserum and was the apparent source of the specific serum immunoglobulin .
	manualset3
136576	5	407536	13	NULL	NULL	0	NULL	intracellular staining 	Research Activity												NULL		0	NULL	NULL	NULL	NULL	NULL	A population of plasma cells was also identified in the peripheral blood of patient Ei that showed strong intracellular staining with the idiotypic antiserum and was the apparent source of the specific serum immunoglobulin .
	manualset3
136577	6	407536	13	NULL	NULL	0	NULL	idiotypic antiserum 	Body part												NULL		0	NULL	NULL	NULL	NULL	NULL	A population of plasma cells was also identified in the peripheral blood of patient Ei that showed strong intracellular staining with the idiotypic antiserum and was the apparent source of the specific serum immunoglobulin .
	manualset3
136578	7	407536	13	NULL	NULL	0	NULL	source 	Body part												NULL		0	NULL	NULL	NULL	NULL	NULL	A population of plasma cells was also identified in the peripheral blood of patient Ei that showed strong intracellular staining with the idiotypic antiserum and was the apparent source of the specific serum immunoglobulin .
	manualset3
136579	8	407536	13	NULL	NULL	0	NULL	serum immunoglobulin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A population of plasma cells was also identified in the peripheral blood of patient Ei that showed strong intracellular staining with the idiotypic antiserum and was the apparent source of the specific serum immunoglobulin .
	manualset3
136580	1	407537	13	NULL	NULL	0	NULL	Structural studies 	Research Activty												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural studies of phosphoglucose isomerase from Mycobacterium tuberculosis H37Rv .
	manualset3
136581	2	407537	13	NULL	NULL	0	NULL	phosphoglucose isomerase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural studies of phosphoglucose isomerase from Mycobacterium tuberculosis H37Rv .
	manualset3
136582	3	407537	13	NULL	NULL	0	NULL	Mycobacterium tuberculosis H37Rv 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural studies of phosphoglucose isomerase from Mycobacterium tuberculosis H37Rv .
	manualset3
136583	1	407538	13	NULL	NULL	0	NULL	Structural variations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural variations of bis-Nts appeared to be dependent on a bis-Nt-OLIG binding constant and were found to be small in the specific DNA binding and highest for nonspecific binding of bis-Nt with the corresponding OLIG .
	manualset3
136584	2	407538	13	NULL	NULL	0	NULL	bis-Nts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural variations of bis-Nts appeared to be dependent on a bis-Nt-OLIG binding constant and were found to be small in the specific DNA binding and highest for nonspecific binding of bis-Nt with the corresponding OLIG .
	manualset3
136585	3	407538	13	NULL	NULL	0	NULL	bis-Nt-OLIG binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural variations of bis-Nts appeared to be dependent on a bis-Nt-OLIG binding constant and were found to be small in the specific DNA binding and highest for nonspecific binding of bis-Nt with the corresponding OLIG .
	manualset3
136586	4	407538	13	NULL	NULL	0	NULL	DNA binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural variations of bis-Nts appeared to be dependent on a bis-Nt-OLIG binding constant and were found to be small in the specific DNA binding and highest for nonspecific binding of bis-Nt with the corresponding OLIG .
	manualset3
136587	5	407538	13	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural variations of bis-Nts appeared to be dependent on a bis-Nt-OLIG binding constant and were found to be small in the specific DNA binding and highest for nonspecific binding of bis-Nt with the corresponding OLIG .
	manualset3
136588	6	407538	13	NULL	NULL	0	NULL	bis-Nt 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural variations of bis-Nts appeared to be dependent on a bis-Nt-OLIG binding constant and were found to be small in the specific DNA binding and highest for nonspecific binding of bis-Nt with the corresponding OLIG .
	manualset3
136589	7	407538	13	NULL	NULL	0	NULL	OLIG	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural variations of bis-Nts appeared to be dependent on a bis-Nt-OLIG binding constant and were found to be small in the specific DNA binding and highest for nonspecific binding of bis-Nt with the corresponding OLIG .
	manualset3
136590	1	407539	13	NULL	NULL	0	NULL	Structure-3A4 MDI relationship studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure-3A4 MDI relationship studies culminated in the discovery of a difluoro analog , ( S ) - N - ( 1 - ( 4-fluoro-3-morpholin-4-ylphenyl ) ethyl ) -3 - ( 4-fluoro-phenyl ) acrylamide ( 2 ) , as an orally bioavailable KCNQ2 opener free of CYP3A4 MDI .
	manualset3
136591	2	407539	13	NULL	NULL	0	NULL	discovery	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure-3A4 MDI relationship studies culminated in the discovery of a difluoro analog , ( S ) - N - ( 1 - ( 4-fluoro-3-morpholin-4-ylphenyl ) ethyl ) -3 - ( 4-fluoro-phenyl ) acrylamide ( 2 ) , as an orally bioavailable KCNQ2 opener free of CYP3A4 MDI .
	manualset3
136592	3	407539	13	NULL	NULL	0	NULL	difluoro analog	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure-3A4 MDI relationship studies culminated in the discovery of a difluoro analog , ( S ) - N - ( 1 - ( 4-fluoro-3-morpholin-4-ylphenyl ) ethyl ) -3 - ( 4-fluoro-phenyl ) acrylamide ( 2 ) , as an orally bioavailable KCNQ2 opener free of CYP3A4 MDI .
	manualset3
136593	4	407539	13	NULL	NULL	0	NULL	( S ) - N - ( 1 - ( 4-fluoro-3-morpholin-4-ylphenyl ) ethyl ) -3 - ( 4-fluoro-phenyl ) acrylamide ( 2 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure-3A4 MDI relationship studies culminated in the discovery of a difluoro analog , ( S ) - N - ( 1 - ( 4-fluoro-3-morpholin-4-ylphenyl ) ethyl ) -3 - ( 4-fluoro-phenyl ) acrylamide ( 2 ) , as an orally bioavailable KCNQ2 opener free of CYP3A4 MDI .
	manualset3
136594	5	407539	13	NULL	NULL	0	NULL	KCNQ2 opener	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure-3A4 MDI relationship studies culminated in the discovery of a difluoro analog , ( S ) - N - ( 1 - ( 4-fluoro-3-morpholin-4-ylphenyl ) ethyl ) -3 - ( 4-fluoro-phenyl ) acrylamide ( 2 ) , as an orally bioavailable KCNQ2 opener free of CYP3A4 MDI .
	manualset3
136595	6	407539	13	NULL	NULL	0	NULL	CYP3A4 MDI	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure-3A4 MDI relationship studies culminated in the discovery of a difluoro analog , ( S ) - N - ( 1 - ( 4-fluoro-3-morpholin-4-ylphenyl ) ethyl ) -3 - ( 4-fluoro-phenyl ) acrylamide ( 2 ) , as an orally bioavailable KCNQ2 opener free of CYP3A4 MDI .
	manualset3
136596	1	407540	13	NULL	NULL	0	NULL	Structure-activity relationships ( SAR ) 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure-activity relationships ( SAR ) and molecular modeling led to the development of a more potent and selective kappa antagonist ( 5 ' - guanidinylnaltrindole , GNTI ) .
	manualset3
136597	2	407540	13	NULL	NULL	0	NULL	molecular modeling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure-activity relationships ( SAR ) and molecular modeling led to the development of a more potent and selective kappa antagonist ( 5 ' - guanidinylnaltrindole , GNTI ) .
	manualset3
136598	3	407540	13	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure-activity relationships ( SAR ) and molecular modeling led to the development of a more potent and selective kappa antagonist ( 5 ' - guanidinylnaltrindole , GNTI ) .
	manualset3
136599	4	407540	13	NULL	NULL	0	NULL	kappa antagonist ( 5 ' - guanidinylnaltrindole , GNTI )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure-activity relationships ( SAR ) and molecular modeling led to the development of a more potent and selective kappa antagonist ( 5 ' - guanidinylnaltrindole , GNTI ) .
	manualset3
136600	1	407541	13	NULL	NULL	0	NULL	Structure-activity relationships 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure-activity relationships , ligand efficiency , and lipophilic efficiency profiles of benzophenone-type inhibitors of the multidrug transporter p-glycoprotein .
	manualset3
136601	2	407541	13	NULL	NULL	0	NULL	ligand efficiency	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure-activity relationships , ligand efficiency , and lipophilic efficiency profiles of benzophenone-type inhibitors of the multidrug transporter p-glycoprotein .
	manualset3
136602	3	407541	13	NULL	NULL	0	NULL	lipophilic efficiency profiles	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure-activity relationships , ligand efficiency , and lipophilic efficiency profiles of benzophenone-type inhibitors of the multidrug transporter p-glycoprotein .
	manualset3
136603	4	407541	13	NULL	NULL	0	NULL	benzophenone-type inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure-activity relationships , ligand efficiency , and lipophilic efficiency profiles of benzophenone-type inhibitors of the multidrug transporter p-glycoprotein .
	manualset3
136604	5	407541	13	NULL	NULL	0	NULL	multidrug transporter p-glycoprotein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure-activity relationships , ligand efficiency , and lipophilic efficiency profiles of benzophenone-type inhibitors of the multidrug transporter p-glycoprotein .
	manualset3
136605	1	407542	13	NULL	NULL	0	NULL	Structure-antifungal activity relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure-antifungal activity relationship of cinnamic acid derivatives .
	manualset3
136606	2	407542	13	NULL	NULL	0	NULL	cinnamic acid derivatives	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure-antifungal activity relationship of cinnamic acid derivatives .
	manualset3
136607	1	407543	13	NULL	NULL	NULL	NULL	Structure	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Structure , function , clinical implications , and phylogeny are reviewed .
	manualset3
136608	2	407543	13	NULL	NULL	NULL	NULL	function	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Structure , function , clinical implications , and phylogeny are reviewed .
	manualset3
136609	3	407543	13	NULL	NULL	0	NULL	clinical implications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure , function , clinical implications , and phylogeny are reviewed .
	manualset3
136610	4	407543	13	NULL	NULL	0	NULL	phylogeny	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure , function , clinical implications , and phylogeny are reviewed .
	manualset3
136611	1	407544	13	NULL	NULL	0	NULL	Structure	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure and biosynthesis of free lipid A molecules that replace lipopolysaccharide in Francisella tularensis subsp .
	manualset3
136612	2	407544	13	NULL	NULL	0	NULL	biosynthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure and biosynthesis of free lipid A molecules that replace lipopolysaccharide in Francisella tularensis subsp .
	manualset3
136613	3	407544	13	NULL	NULL	0	NULL	 lipid A molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure and biosynthesis of free lipid A molecules that replace lipopolysaccharide in Francisella tularensis subsp .
	manualset3
136614	4	407544	13	NULL	NULL	0	NULL	lipopolysaccharide	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure and biosynthesis of free lipid A molecules that replace lipopolysaccharide in Francisella tularensis subsp .
	manualset3
136615	5	407544	13	NULL	NULL	0	NULL	Francisella tularensis subsp	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure and biosynthesis of free lipid A molecules that replace lipopolysaccharide in Francisella tularensis subsp .
	manualset3
136616	1	407545	13	NULL	NULL	0	NULL	Structure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure and mechanism of formation of the two forms of 18-hydroxy-11-deoxycorticosterone .
	manualset3
136617	2	407545	13	NULL	NULL	0	NULL	mechanism of formation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure and mechanism of formation of the two forms of 18-hydroxy-11-deoxycorticosterone .
	manualset3
136618	3	407545	13	NULL	NULL	0	NULL	two forms	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure and mechanism of formation of the two forms of 18-hydroxy-11-deoxycorticosterone .
	manualset3
136619	4	407545	13	NULL	NULL	0	NULL	18-hydroxy-11-deoxycorticosterone 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure and mechanism of formation of the two forms of 18-hydroxy-11-deoxycorticosterone .
	manualset3
136620	1	407546	13	NULL	NULL	0	NULL	Change	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Change in the cardiac contraction phase in patients with hypertension under the effect of intraventricular administration of oxygen ) .
	manualset3
136621	2	407546	13	NULL	NULL	0	NULL	cardiac contraction phase	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Change in the cardiac contraction phase in patients with hypertension under the effect of intraventricular administration of oxygen ) .
	manualset3
136622	3	407546	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Change in the cardiac contraction phase in patients with hypertension under the effect of intraventricular administration of oxygen ) .
	manualset3
136623	4	407546	13	NULL	NULL	0	NULL	hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Change in the cardiac contraction phase in patients with hypertension under the effect of intraventricular administration of oxygen ) .
	manualset3
136624	5	407546	13	NULL	NULL	0	NULL	effect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Change in the cardiac contraction phase in patients with hypertension under the effect of intraventricular administration of oxygen ) .
	manualset3
136625	6	407546	13	NULL	NULL	0	NULL	intraventricular administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Change in the cardiac contraction phase in patients with hypertension under the effect of intraventricular administration of oxygen ) .
	manualset3
136626	7	407546	13	NULL	NULL	0	NULL	oxygen	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	( Change in the cardiac contraction phase in patients with hypertension under the effect of intraventricular administration of oxygen ) .
	manualset3
136627	1	407547	13	NULL	NULL	0	NULL	population survey	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A population survey of the penetrance of contact lens wear in Australia : rationale , methodology and results .
	manualset3
136628	2	407547	13	NULL	NULL	0	NULL	penetrance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A population survey of the penetrance of contact lens wear in Australia : rationale , methodology and results .
	manualset3
136629	3	407547	13	NULL	NULL	0	NULL	contact lens wear 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A population survey of the penetrance of contact lens wear in Australia : rationale , methodology and results .
	manualset3
136630	4	407547	13	NULL	NULL	0	NULL	Australia 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A population survey of the penetrance of contact lens wear in Australia : rationale , methodology and results .
	manualset3
136631	5	407547	13	NULL	NULL	0	NULL	rationale	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A population survey of the penetrance of contact lens wear in Australia : rationale , methodology and results .
	manualset3
136632	6	407547	13	NULL	NULL	0	NULL	methodology 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A population survey of the penetrance of contact lens wear in Australia : rationale , methodology and results .
	manualset3
136633	7	407547	13	NULL	NULL	0	NULL	results	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A population survey of the penetrance of contact lens wear in Australia : rationale , methodology and results .
	manualset3
136634	1	407548	13	NULL	NULL	0	NULL	Structure	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure and sequence of the chicken type II procollagen gene .
	manualset3
136635	2	407548	13	NULL	NULL	0	NULL	sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure and sequence of the chicken type II procollagen gene .
	manualset3
136636	3	407548	13	NULL	NULL	0	NULL	chicken type II procollagen gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure and sequence of the chicken type II procollagen gene .
	manualset3
136637	1	407549	13	NULL	NULL	0	NULL	Structure	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure guided approaches toward exploiting and manipulating nonribosomal peptide and polyketide biosynthetic pathways .
	manualset3
136638	2	407549	13	NULL	NULL	NULL	NULL	approaches	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Structure guided approaches toward exploiting and manipulating nonribosomal peptide and polyketide biosynthetic pathways .
	manualset3
136639	3	407549	13	NULL	NULL	0	NULL	nonribosomal peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure guided approaches toward exploiting and manipulating nonribosomal peptide and polyketide biosynthetic pathways .
	manualset3
136640	4	407549	13	NULL	NULL	0	NULL	polyketide biosynthetic pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure guided approaches toward exploiting and manipulating nonribosomal peptide and polyketide biosynthetic pathways .
	manualset3
136641	1	407550	13	NULL	NULL	0	NULL	Student 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Student response to teaching and learning in the simulator over a 3-year evaluation period , collected via a student questionnaire was uniformly positive .
	manualset3
136642	2	407550	13	NULL	NULL	0	NULL	response 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Student response to teaching and learning in the simulator over a 3-year evaluation period , collected via a student questionnaire was uniformly positive .
	manualset3
136643	3	407550	13	NULL	NULL	0	NULL	 teaching	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Student response to teaching and learning in the simulator over a 3-year evaluation period , collected via a student questionnaire was uniformly positive .
	manualset3
136644	4	407550	13	NULL	NULL	0	NULL	learning 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Student response to teaching and learning in the simulator over a 3-year evaluation period , collected via a student questionnaire was uniformly positive .
	manualset3
136645	5	407550	13	NULL	NULL	0	NULL	simulator	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Student response to teaching and learning in the simulator over a 3-year evaluation period , collected via a student questionnaire was uniformly positive .
	manualset3
136646	6	407550	13	NULL	NULL	0	NULL	3-year evaluation period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Student response to teaching and learning in the simulator over a 3-year evaluation period , collected via a student questionnaire was uniformly positive .
	manualset3
136647	7	407550	13	NULL	NULL	0	NULL	student questionnaire	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Student response to teaching and learning in the simulator over a 3-year evaluation period , collected via a student questionnaire was uniformly positive .
	manualset3
136648	1	407551	13	NULL	NULL	0	NULL	Students '	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Students ' perspectives of effective and ineffective nursing instructors .
	manualset3
136649	2	407551	13	NULL	NULL	0	NULL	perspectives	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Students ' perspectives of effective and ineffective nursing instructors .
	manualset3
136650	3	407551	13	NULL	NULL	0	NULL	 instructors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Students ' perspectives of effective and ineffective nursing instructors .
	manualset3
136651	1	407552	13	NULL	NULL	0	NULL	Students	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Students lived in the hospital in available patient rooms for that week .
	manualset3
136652	2	407552	13	NULL	NULL	0	NULL	hospital	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Students lived in the hospital in available patient rooms for that week .
	manualset3
136653	3	407552	13	NULL	NULL	0	NULL	patient rooms	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Students lived in the hospital in available patient rooms for that week .
	manualset3
136654	4	407552	13	NULL	NULL	0	NULL	week	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Students lived in the hospital in available patient rooms for that week .
	manualset3
136655	1	407553	13	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies evaluating the efficacy of combined analgesia have demonstrated significant benefits for combinations of 2 or more forms of treatment ( such as DPNB and sucrose-dipped pacifier ) compared with single interventions .
	manualset3
136656	2	407553	13	NULL	NULL	0	NULL	efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies evaluating the efficacy of combined analgesia have demonstrated significant benefits for combinations of 2 or more forms of treatment ( such as DPNB and sucrose-dipped pacifier ) compared with single interventions .
	manualset3
136657	3	407553	13	NULL	NULL	0	NULL	analgesia	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies evaluating the efficacy of combined analgesia have demonstrated significant benefits for combinations of 2 or more forms of treatment ( such as DPNB and sucrose-dipped pacifier ) compared with single interventions .
	manualset3
136658	4	407553	13	NULL	NULL	0	NULL	benefits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies evaluating the efficacy of combined analgesia have demonstrated significant benefits for combinations of 2 or more forms of treatment ( such as DPNB and sucrose-dipped pacifier ) compared with single interventions .
	manualset3
136659	5	407553	13	NULL	NULL	0	NULL	combinations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies evaluating the efficacy of combined analgesia have demonstrated significant benefits for combinations of 2 or more forms of treatment ( such as DPNB and sucrose-dipped pacifier ) compared with single interventions .
	manualset3
136660	6	407553	13	NULL	NULL	0	NULL	2 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies evaluating the efficacy of combined analgesia have demonstrated significant benefits for combinations of 2 or more forms of treatment ( such as DPNB and sucrose-dipped pacifier ) compared with single interventions .
	manualset3
136661	7	407553	13	NULL	NULL	NULL	NULL	forms of treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Studies evaluating the efficacy of combined analgesia have demonstrated significant benefits for combinations of 2 or more forms of treatment ( such as DPNB and sucrose-dipped pacifier ) compared with single interventions .
	manualset3
136662	8	407553	13	NULL	NULL	0	NULL	DPNB	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies evaluating the efficacy of combined analgesia have demonstrated significant benefits for combinations of 2 or more forms of treatment ( such as DPNB and sucrose-dipped pacifier ) compared with single interventions .
	manualset3
136663	9	407553	13	NULL	NULL	0	NULL	sucrose-dipped pacifier	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies evaluating the efficacy of combined analgesia have demonstrated significant benefits for combinations of 2 or more forms of treatment ( such as DPNB and sucrose-dipped pacifier ) compared with single interventions .
	manualset3
136664	10	407553	13	NULL	NULL	0	NULL	single interventions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies evaluating the efficacy of combined analgesia have demonstrated significant benefits for combinations of 2 or more forms of treatment ( such as DPNB and sucrose-dipped pacifier ) compared with single interventions .
	manualset3
136665	1	407554	13	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies from model systems have demonstrated that palindrome formation can be an early step in DNA amplification , most notably seen in the breakage-fusion-bridge ( BFB ) cycle .
	manualset3
136666	2	407554	13	NULL	NULL	0	NULL	model systems	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies from model systems have demonstrated that palindrome formation can be an early step in DNA amplification , most notably seen in the breakage-fusion-bridge ( BFB ) cycle .
	manualset3
136667	3	407554	13	NULL	NULL	0	NULL	palindrome formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies from model systems have demonstrated that palindrome formation can be an early step in DNA amplification , most notably seen in the breakage-fusion-bridge ( BFB ) cycle .
	manualset3
136668	4	407554	13	NULL	NULL	0	NULL	early step	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies from model systems have demonstrated that palindrome formation can be an early step in DNA amplification , most notably seen in the breakage-fusion-bridge ( BFB ) cycle .
	manualset3
136669	5	407554	13	NULL	NULL	0	NULL	DNA amplification 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies from model systems have demonstrated that palindrome formation can be an early step in DNA amplification , most notably seen in the breakage-fusion-bridge ( BFB ) cycle .
	manualset3
136670	6	407554	13	NULL	NULL	0	NULL	breakage-fusion-bridge ( BFB ) cycle	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies from model systems have demonstrated that palindrome formation can be an early step in DNA amplification , most notably seen in the breakage-fusion-bridge ( BFB ) cycle .
	manualset3
136671	1	407555	13	NULL	NULL	0	NULL	Studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have already demonstrated the benefits of applying gene expression profiling towards drug safety evaluation , both for identifying mechanisms underlying toxicity , as well as for providing a means to identify safety liabilities early in the drug discovery process .
	manualset3
136672	2	407555	13	NULL	NULL	0	NULL	benefits 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have already demonstrated the benefits of applying gene expression profiling towards drug safety evaluation , both for identifying mechanisms underlying toxicity , as well as for providing a means to identify safety liabilities early in the drug discovery process .
	manualset3
136673	3	407555	13	NULL	NULL	0	NULL	gene expression profiling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have already demonstrated the benefits of applying gene expression profiling towards drug safety evaluation , both for identifying mechanisms underlying toxicity , as well as for providing a means to identify safety liabilities early in the drug discovery process .
	manualset3
136674	4	407555	13	NULL	NULL	0	NULL	drug safety evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have already demonstrated the benefits of applying gene expression profiling towards drug safety evaluation , both for identifying mechanisms underlying toxicity , as well as for providing a means to identify safety liabilities early in the drug discovery process .
	manualset3
136675	5	407555	13	NULL	NULL	0	NULL	mechanisms 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have already demonstrated the benefits of applying gene expression profiling towards drug safety evaluation , both for identifying mechanisms underlying toxicity , as well as for providing a means to identify safety liabilities early in the drug discovery process .
	manualset3
136676	6	407555	13	NULL	NULL	0	NULL	toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have already demonstrated the benefits of applying gene expression profiling towards drug safety evaluation , both for identifying mechanisms underlying toxicity , as well as for providing a means to identify safety liabilities early in the drug discovery process .
	manualset3
136677	7	407555	13	NULL	NULL	0	NULL	means	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have already demonstrated the benefits of applying gene expression profiling towards drug safety evaluation , both for identifying mechanisms underlying toxicity , as well as for providing a means to identify safety liabilities early in the drug discovery process .
	manualset3
136678	8	407555	13	NULL	NULL	0	NULL	safety liabilities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have already demonstrated the benefits of applying gene expression profiling towards drug safety evaluation , both for identifying mechanisms underlying toxicity , as well as for providing a means to identify safety liabilities early in the drug discovery process .
	manualset3
136679	9	407555	13	NULL	NULL	0	NULL	drug discovery process 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have already demonstrated the benefits of applying gene expression profiling towards drug safety evaluation , both for identifying mechanisms underlying toxicity , as well as for providing a means to identify safety liabilities early in the drug discovery process .
	manualset3
136680	1	407556	13	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have been carried out both in culture and in vivo to examine the mechanism of action of fazarabine in P388 murine and Molt-4 human lymphoblasts .
	manualset3
136682	2	407556	13	NULL	NULL	0	NULL	culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have been carried out both in culture and in vivo to examine the mechanism of action of fazarabine in P388 murine and Molt-4 human lymphoblasts .
	manualset3
136683	3	407556	13	NULL	NULL	0	NULL	mechanism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have been carried out both in culture and in vivo to examine the mechanism of action of fazarabine in P388 murine and Molt-4 human lymphoblasts .
	manualset3
136686	4	407556	13	NULL	NULL	0	NULL	action	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have been carried out both in culture and in vivo to examine the mechanism of action of fazarabine in P388 murine and Molt-4 human lymphoblasts .
	manualset3
136688	5	407556	13	NULL	NULL	0	NULL	fazarabine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have been carried out both in culture and in vivo to examine the mechanism of action of fazarabine in P388 murine and Molt-4 human lymphoblasts .
	manualset3
136689	6	407556	13	NULL	NULL	0	NULL	P388 murine lymphoblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have been carried out both in culture and in vivo to examine the mechanism of action of fazarabine in P388 murine and Molt-4 human lymphoblasts .
	manualset3
136690	7	407556	13	NULL	NULL	0	NULL	Molt-4 human lymphoblasts 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have been carried out both in culture and in vivo to examine the mechanism of action of fazarabine in P388 murine and Molt-4 human lymphoblasts .
	manualset3
136692	1	407557	13	NULL	NULL	0	NULL	porcine model	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A porcine model of acute lung injury was used to provide recordings of different respiratory mechanics conditions .
	manualset3
136693	2	407557	13	NULL	NULL	0	NULL	acute lung injury 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A porcine model of acute lung injury was used to provide recordings of different respiratory mechanics conditions .
	manualset3
136694	3	407557	13	NULL	NULL	0	NULL	recordings 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A porcine model of acute lung injury was used to provide recordings of different respiratory mechanics conditions .
	manualset3
136695	4	407557	13	NULL	NULL	0	NULL	respiratory mechanics conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A porcine model of acute lung injury was used to provide recordings of different respiratory mechanics conditions .
	manualset3
136696	1	407558	13	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have been made in 1407 patients of the causes , the organs involved and the outcome of injury to the abdomen in patients needing admission to hospital in an area of Southern Sweden , between 1950 and the end of 1979 .
	manualset3
136697	2	407558	13	NULL	NULL	0	NULL	1407 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have been made in 1407 patients of the causes , the organs involved and the outcome of injury to the abdomen in patients needing admission to hospital in an area of Southern Sweden , between 1950 and the end of 1979 .
	manualset3
136698	3	407558	13	NULL	NULL	0	NULL	causes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have been made in 1407 patients of the causes , the organs involved and the outcome of injury to the abdomen in patients needing admission to hospital in an area of Southern Sweden , between 1950 and the end of 1979 .
	manualset3
136699	4	407558	13	NULL	NULL	0	NULL	organs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have been made in 1407 patients of the causes , the organs involved and the outcome of injury to the abdomen in patients needing admission to hospital in an area of Southern Sweden , between 1950 and the end of 1979 .
	manualset3
136700	5	407558	13	NULL	NULL	0	NULL	outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have been made in 1407 patients of the causes , the organs involved and the outcome of injury to the abdomen in patients needing admission to hospital in an area of Southern Sweden , between 1950 and the end of 1979 .
	manualset3
136701	6	407558	13	NULL	NULL	0	NULL	injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have been made in 1407 patients of the causes , the organs involved and the outcome of injury to the abdomen in patients needing admission to hospital in an area of Southern Sweden , between 1950 and the end of 1979 .
	manualset3
136702	7	407558	13	NULL	NULL	0	NULL	abdomen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have been made in 1407 patients of the causes , the organs involved and the outcome of injury to the abdomen in patients needing admission to hospital in an area of Southern Sweden , between 1950 and the end of 1979 .
	manualset3
136703	8	407558	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have been made in 1407 patients of the causes , the organs involved and the outcome of injury to the abdomen in patients needing admission to hospital in an area of Southern Sweden , between 1950 and the end of 1979 .
	manualset3
136704	9	407558	13	NULL	NULL	0	NULL	admission	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have been made in 1407 patients of the causes , the organs involved and the outcome of injury to the abdomen in patients needing admission to hospital in an area of Southern Sweden , between 1950 and the end of 1979 .
	manualset3
136705	10	407558	13	NULL	NULL	0	NULL	hospital	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have been made in 1407 patients of the causes , the organs involved and the outcome of injury to the abdomen in patients needing admission to hospital in an area of Southern Sweden , between 1950 and the end of 1979 .
	manualset3
136706	11	407558	13	NULL	NULL	0	NULL	area of Southern Sweden	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have been made in 1407 patients of the causes , the organs involved and the outcome of injury to the abdomen in patients needing admission to hospital in an area of Southern Sweden , between 1950 and the end of 1979 .
	manualset3
136707	12	407558	13	NULL	NULL	0	NULL	1950 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have been made in 1407 patients of the causes , the organs involved and the outcome of injury to the abdomen in patients needing admission to hospital in an area of Southern Sweden , between 1950 and the end of 1979 .
	manualset3
136708	13	407558	13	NULL	NULL	0	NULL	1979	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have been made in 1407 patients of the causes , the organs involved and the outcome of injury to the abdomen in patients needing admission to hospital in an area of Southern Sweden , between 1950 and the end of 1979 .
	manualset3
136997	1	407559	13	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have questioned whether renal dysfunction in sickle cell disease is linked to hemolysis-associated vasculopathy .
	manualset3
136998	2	407559	13	NULL	NULL	0	NULL	renal dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have questioned whether renal dysfunction in sickle cell disease is linked to hemolysis-associated vasculopathy .
	manualset3
136999	3	407559	13	NULL	NULL	0	NULL	sickle cell disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have questioned whether renal dysfunction in sickle cell disease is linked to hemolysis-associated vasculopathy .
	manualset3
137000	4	407559	13	NULL	NULL	0	NULL	hemolysis-associated vasculopathy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies have questioned whether renal dysfunction in sickle cell disease is linked to hemolysis-associated vasculopathy .
	manualset3
137001	1	407560	13	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies in carcinogenesis with azo compounds ; the action of four azo dyes in mixed and pure strain mice .
	manualset3
137002	2	407560	13	NULL	NULL	0	NULL	carcinogenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies in carcinogenesis with azo compounds ; the action of four azo dyes in mixed and pure strain mice .
	manualset3
137003	3	407560	13	NULL	NULL	0	NULL	azo compounds 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies in carcinogenesis with azo compounds ; the action of four azo dyes in mixed and pure strain mice .
	manualset3
137004	4	407560	13	NULL	NULL	0	NULL	action 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies in carcinogenesis with azo compounds ; the action of four azo dyes in mixed and pure strain mice .
	manualset3
137005	5	407560	13	NULL	NULL	0	NULL	four azo dyes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies in carcinogenesis with azo compounds ; the action of four azo dyes in mixed and pure strain mice .
	manualset3
137006	6	407560	13	NULL	NULL	0	NULL	mixed strain mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies in carcinogenesis with azo compounds ; the action of four azo dyes in mixed and pure strain mice .
	manualset3
137007	7	407560	13	NULL	NULL	0	NULL	pure strain mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies in carcinogenesis with azo compounds ; the action of four azo dyes in mixed and pure strain mice .
	manualset3
137008	1	407561	13	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies in the U.S. have shown that use of stilbestrol during pregnancy can cause vaginal cancer in female offspring during and after puberty .
	manualset3
137009	2	407561	13	NULL	NULL	0	NULL	U.S. 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies in the U.S. have shown that use of stilbestrol during pregnancy can cause vaginal cancer in female offspring during and after puberty .
	manualset3
137010	3	407561	13	NULL	NULL	0	NULL	use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies in the U.S. have shown that use of stilbestrol during pregnancy can cause vaginal cancer in female offspring during and after puberty .
	manualset3
137011	4	407561	13	NULL	NULL	0	NULL	stilbestrol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies in the U.S. have shown that use of stilbestrol during pregnancy can cause vaginal cancer in female offspring during and after puberty .
	manualset3
137012	5	407561	13	NULL	NULL	0	NULL	pregnancy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies in the U.S. have shown that use of stilbestrol during pregnancy can cause vaginal cancer in female offspring during and after puberty .
	manualset3
137013	6	407561	13	NULL	NULL	0	NULL	vaginal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies in the U.S. have shown that use of stilbestrol during pregnancy can cause vaginal cancer in female offspring during and after puberty .
	manualset3
137014	7	407561	13	NULL	NULL	0	NULL	female offspring 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies in the U.S. have shown that use of stilbestrol during pregnancy can cause vaginal cancer in female offspring during and after puberty .
	manualset3
137015	8	407561	13	NULL	NULL	0	NULL	puberty	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies in the U.S. have shown that use of stilbestrol during pregnancy can cause vaginal cancer in female offspring during and after puberty .
	manualset3
137016	1	407562	13	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies in the pathogenesis and functional regulation of pituitary adenomas are mainly focused on the following two topics : ( a ) the origin of pituitary adenomas and abnormal physical adjustment due to the activation of oncogenes and loss of function for tumour-suppressor genes ; and ( b ) the mechanistic anomalies of the intracellular signal transduction .
	manualset3
137017	2	407562	13	NULL	NULL	0	NULL	pathogenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies in the pathogenesis and functional regulation of pituitary adenomas are mainly focused on the following two topics : ( a ) the origin of pituitary adenomas and abnormal physical adjustment due to the activation of oncogenes and loss of function for tumour-suppressor genes ; and ( b ) the mechanistic anomalies of the intracellular signal transduction .
	manualset3
137018	3	407562	13	NULL	NULL	0	NULL	functional regulation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies in the pathogenesis and functional regulation of pituitary adenomas are mainly focused on the following two topics : ( a ) the origin of pituitary adenomas and abnormal physical adjustment due to the activation of oncogenes and loss of function for tumour-suppressor genes ; and ( b ) the mechanistic anomalies of the intracellular signal transduction .
	manualset3
137019	4	407562	13	NULL	NULL	0	NULL	pituitary adenomas 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies in the pathogenesis and functional regulation of pituitary adenomas are mainly focused on the following two topics : ( a ) the origin of pituitary adenomas and abnormal physical adjustment due to the activation of oncogenes and loss of function for tumour-suppressor genes ; and ( b ) the mechanistic anomalies of the intracellular signal transduction .
	manualset3
137020	5	407562	13	NULL	NULL	0	NULL	two topics 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies in the pathogenesis and functional regulation of pituitary adenomas are mainly focused on the following two topics : ( a ) the origin of pituitary adenomas and abnormal physical adjustment due to the activation of oncogenes and loss of function for tumour-suppressor genes ; and ( b ) the mechanistic anomalies of the intracellular signal transduction .
	manualset3
137021	6	407562	13	NULL	NULL	0	NULL	origin of pituitary adenomas 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies in the pathogenesis and functional regulation of pituitary adenomas are mainly focused on the following two topics : ( a ) the origin of pituitary adenomas and abnormal physical adjustment due to the activation of oncogenes and loss of function for tumour-suppressor genes ; and ( b ) the mechanistic anomalies of the intracellular signal transduction .
	manualset3
137022	7	407562	13	NULL	NULL	0	NULL	abnormal physical adjustment 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies in the pathogenesis and functional regulation of pituitary adenomas are mainly focused on the following two topics : ( a ) the origin of pituitary adenomas and abnormal physical adjustment due to the activation of oncogenes and loss of function for tumour-suppressor genes ; and ( b ) the mechanistic anomalies of the intracellular signal transduction .
	manualset3
137023	8	407562	13	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies in the pathogenesis and functional regulation of pituitary adenomas are mainly focused on the following two topics : ( a ) the origin of pituitary adenomas and abnormal physical adjustment due to the activation of oncogenes and loss of function for tumour-suppressor genes ; and ( b ) the mechanistic anomalies of the intracellular signal transduction .
	manualset3
137024	9	407562	13	NULL	NULL	0	NULL	oncogenes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies in the pathogenesis and functional regulation of pituitary adenomas are mainly focused on the following two topics : ( a ) the origin of pituitary adenomas and abnormal physical adjustment due to the activation of oncogenes and loss of function for tumour-suppressor genes ; and ( b ) the mechanistic anomalies of the intracellular signal transduction .
	manualset3
137025	10	407562	13	NULL	NULL	0	NULL	loss of function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies in the pathogenesis and functional regulation of pituitary adenomas are mainly focused on the following two topics : ( a ) the origin of pituitary adenomas and abnormal physical adjustment due to the activation of oncogenes and loss of function for tumour-suppressor genes ; and ( b ) the mechanistic anomalies of the intracellular signal transduction .
	manualset3
137026	11	407562	13	NULL	NULL	0	NULL	tumour-suppressor genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies in the pathogenesis and functional regulation of pituitary adenomas are mainly focused on the following two topics : ( a ) the origin of pituitary adenomas and abnormal physical adjustment due to the activation of oncogenes and loss of function for tumour-suppressor genes ; and ( b ) the mechanistic anomalies of the intracellular signal transduction .
	manualset3
137027	12	407562	13	NULL	NULL	0	NULL	mechanistic anomalies	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies in the pathogenesis and functional regulation of pituitary adenomas are mainly focused on the following two topics : ( a ) the origin of pituitary adenomas and abnormal physical adjustment due to the activation of oncogenes and loss of function for tumour-suppressor genes ; and ( b ) the mechanistic anomalies of the intracellular signal transduction .
	manualset3
137028	13	407562	13	NULL	NULL	0	NULL	intracellular signal transduction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies in the pathogenesis and functional regulation of pituitary adenomas are mainly focused on the following two topics : ( a ) the origin of pituitary adenomas and abnormal physical adjustment due to the activation of oncogenes and loss of function for tumour-suppressor genes ; and ( b ) the mechanistic anomalies of the intracellular signal transduction .
	manualset3
137029	1	407563	13	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies included 50 males : 20 patients with intermittent claudication , 10 patients with chronic cardiac failure , and 10 patients with varicose veins .
	manualset3
137030	2	407563	13	NULL	NULL	0	NULL	50 males	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies included 50 males : 20 patients with intermittent claudication , 10 patients with chronic cardiac failure , and 10 patients with varicose veins .
	manualset3
137031	3	407563	13	NULL	NULL	0	NULL	 20 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies included 50 males : 20 patients with intermittent claudication , 10 patients with chronic cardiac failure , and 10 patients with varicose veins .
	manualset3
137032	4	407563	13	NULL	NULL	0	NULL	 intermittent claudication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies included 50 males : 20 patients with intermittent claudication , 10 patients with chronic cardiac failure , and 10 patients with varicose veins .
	manualset3
137033	5	407563	13	NULL	NULL	0	NULL	10 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies included 50 males : 20 patients with intermittent claudication , 10 patients with chronic cardiac failure , and 10 patients with varicose veins .
	manualset3
137034	6	407563	13	NULL	NULL	0	NULL	 chronic cardiac failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies included 50 males : 20 patients with intermittent claudication , 10 patients with chronic cardiac failure , and 10 patients with varicose veins .
	manualset3
137035	7	407563	13	NULL	NULL	0	NULL	10 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies included 50 males : 20 patients with intermittent claudication , 10 patients with chronic cardiac failure , and 10 patients with varicose veins .
	manualset3
137036	8	407563	13	NULL	NULL	0	NULL	varicose veins	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies included 50 males : 20 patients with intermittent claudication , 10 patients with chronic cardiac failure , and 10 patients with varicose veins .
	manualset3
137037	1	407564	13	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of CD146 expression and function in breast cancer remain scarce .
	manualset3
137038	2	407564	13	NULL	NULL	0	NULL	CD146 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of CD146 expression and function in breast cancer remain scarce .
	manualset3
137039	3	407564	13	NULL	NULL	0	NULL	function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of CD146 expression and function in breast cancer remain scarce .
	manualset3
137040	4	407564	13	NULL	NULL	0	NULL	breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of CD146 expression and function in breast cancer remain scarce .
	manualset3
137041	1	407565	13	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of Slc26a4-null mice indicate that pendrin is essential for inner ear development , but have not revealed whether pendrin is specifically necessary for homeostasis .
	manualset3
137042	2	407565	13	NULL	NULL	0	NULL	Slc26a4-null mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of Slc26a4-null mice indicate that pendrin is essential for inner ear development , but have not revealed whether pendrin is specifically necessary for homeostasis .
	manualset3
137043	3	407565	13	NULL	NULL	0	NULL	pendrin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of Slc26a4-null mice indicate that pendrin is essential for inner ear development , but have not revealed whether pendrin is specifically necessary for homeostasis .
	manualset3
137044	4	407565	13	NULL	NULL	0	NULL	inner ear development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of Slc26a4-null mice indicate that pendrin is essential for inner ear development , but have not revealed whether pendrin is specifically necessary for homeostasis .
	manualset3
137045	5	407565	13	NULL	NULL	0	NULL	pendrin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of Slc26a4-null mice indicate that pendrin is essential for inner ear development , but have not revealed whether pendrin is specifically necessary for homeostasis .
	manualset3
137046	6	407565	13	NULL	NULL	0	NULL	homeostasis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of Slc26a4-null mice indicate that pendrin is essential for inner ear development , but have not revealed whether pendrin is specifically necessary for homeostasis .
	manualset3
137047	1	407566	13	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of aerosol distributions in a small laboratory containing a heated phantom .
	manualset3
137048	2	407566	13	NULL	NULL	0	NULL	aerosol distributions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of aerosol distributions in a small laboratory containing a heated phantom .
	manualset3
137049	3	407566	13	NULL	NULL	0	NULL	small laboratory 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of aerosol distributions in a small laboratory containing a heated phantom .
	manualset3
137050	4	407566	13	NULL	NULL	0	NULL	phantom	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of aerosol distributions in a small laboratory containing a heated phantom .
	manualset3
137051	1	407567	13	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of deep gray structures in AD brains reveal elevated levels of GAL in the nucleus basalis .
	manualset3
137052	2	407567	13	NULL	NULL	0	NULL	deep gray structures	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of deep gray structures in AD brains reveal elevated levels of GAL in the nucleus basalis .
	manualset3
137053	3	407567	13	NULL	NULL	0	NULL	AD brains 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of deep gray structures in AD brains reveal elevated levels of GAL in the nucleus basalis .
	manualset3
137054	4	407567	13	NULL	NULL	0	NULL	levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of deep gray structures in AD brains reveal elevated levels of GAL in the nucleus basalis .
	manualset3
137055	5	407567	13	NULL	NULL	0	NULL	GAL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of deep gray structures in AD brains reveal elevated levels of GAL in the nucleus basalis .
	manualset3
137056	6	407567	13	NULL	NULL	0	NULL	nucleus basalis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of deep gray structures in AD brains reveal elevated levels of GAL in the nucleus basalis .
	manualset3
137057	1	407568	13	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of drug resistance mainly focus on the cellular resistance mechanisms rather than how the cells develop resistance .
	manualset3
137058	2	407568	13	NULL	NULL	0	NULL	drug resistance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of drug resistance mainly focus on the cellular resistance mechanisms rather than how the cells develop resistance .
	manualset3
137059	3	407568	13	NULL	NULL	0	NULL	cellular resistance mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of drug resistance mainly focus on the cellular resistance mechanisms rather than how the cells develop resistance .
	manualset3
137060	4	407568	13	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of drug resistance mainly focus on the cellular resistance mechanisms rather than how the cells develop resistance .
	manualset3
137061	5	407568	13	NULL	NULL	0	NULL	resistance 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of drug resistance mainly focus on the cellular resistance mechanisms rather than how the cells develop resistance .
	manualset3
137062	1	407569	13	NULL	NULL	0	NULL	Studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of genetic and acquired alterations of complement proteins have provided insights into the pathophysiology of a number of rheumatic diseases , especially those in which immune complexes are believed to have a role in pathogenesis .
	manualset3
137063	2	407569	13	NULL	NULL	0	NULL	genetic alterations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of genetic and acquired alterations of complement proteins have provided insights into the pathophysiology of a number of rheumatic diseases , especially those in which immune complexes are believed to have a role in pathogenesis .
	manualset3
137064	3	407569	13	NULL	NULL	0	NULL	acquired alterations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of genetic and acquired alterations of complement proteins have provided insights into the pathophysiology of a number of rheumatic diseases , especially those in which immune complexes are believed to have a role in pathogenesis .
	manualset3
137065	4	407569	13	NULL	NULL	0	NULL	complement proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of genetic and acquired alterations of complement proteins have provided insights into the pathophysiology of a number of rheumatic diseases , especially those in which immune complexes are believed to have a role in pathogenesis .
	manualset3
137066	5	407569	13	NULL	NULL	0	NULL	insights 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of genetic and acquired alterations of complement proteins have provided insights into the pathophysiology of a number of rheumatic diseases , especially those in which immune complexes are believed to have a role in pathogenesis .
	manualset3
137067	6	407569	13	NULL	NULL	0	NULL	pathophysiology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of genetic and acquired alterations of complement proteins have provided insights into the pathophysiology of a number of rheumatic diseases , especially those in which immune complexes are believed to have a role in pathogenesis .
	manualset3
137068	7	407569	13	NULL	NULL	0	NULL	number	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of genetic and acquired alterations of complement proteins have provided insights into the pathophysiology of a number of rheumatic diseases , especially those in which immune complexes are believed to have a role in pathogenesis .
	manualset3
137069	8	407569	13	NULL	NULL	0	NULL	rheumatic diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of genetic and acquired alterations of complement proteins have provided insights into the pathophysiology of a number of rheumatic diseases , especially those in which immune complexes are believed to have a role in pathogenesis .
	manualset3
137070	9	407569	13	NULL	NULL	0	NULL	immune complexes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of genetic and acquired alterations of complement proteins have provided insights into the pathophysiology of a number of rheumatic diseases , especially those in which immune complexes are believed to have a role in pathogenesis .
	manualset3
137071	10	407569	13	NULL	NULL	0	NULL	role in pathogenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of genetic and acquired alterations of complement proteins have provided insights into the pathophysiology of a number of rheumatic diseases , especially those in which immune complexes are believed to have a role in pathogenesis .
	manualset3
137072	1	407570	13	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of liver lobes autotransplanted outside the abdominal cavity .
	manualset3
137073	2	407570	13	NULL	NULL	0	NULL	liver lobes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of liver lobes autotransplanted outside the abdominal cavity .
	manualset3
137074	3	407570	13	NULL	NULL	0	NULL	abdominal cavity	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of liver lobes autotransplanted outside the abdominal cavity .
	manualset3
137075	1	407571	13	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of oogenesis in the rotifer , Asplanchna .
	manualset3
137076	2	407571	13	NULL	NULL	0	NULL	oogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of oogenesis in the rotifer , Asplanchna .
	manualset3
137077	3	407571	13	NULL	NULL	0	NULL	rotifer	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of oogenesis in the rotifer , Asplanchna .
	manualset3
137078	4	407571	13	NULL	NULL	0	NULL	Asplanchna	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of oogenesis in the rotifer , Asplanchna .
	manualset3
137079	1	407572	13	NULL	NULL	0	NULL	Studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of osteosarcoma cell lines or frozen tissue have detected loss of heterozygosity ( LOH ) at the retinoblastoma ( RB ) locus by Southern blot analysis or restriction fragment length polymorphism .
	manualset3
137080	2	407572	13	NULL	NULL	0	NULL	osteosarcoma cell lines 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of osteosarcoma cell lines or frozen tissue have detected loss of heterozygosity ( LOH ) at the retinoblastoma ( RB ) locus by Southern blot analysis or restriction fragment length polymorphism .
	manualset3
137081	3	407572	13	NULL	NULL	0	NULL	frozen tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of osteosarcoma cell lines or frozen tissue have detected loss of heterozygosity ( LOH ) at the retinoblastoma ( RB ) locus by Southern blot analysis or restriction fragment length polymorphism .
	manualset3
137082	4	407572	13	NULL	NULL	0	NULL	loss of heterozygosity ( LOH )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of osteosarcoma cell lines or frozen tissue have detected loss of heterozygosity ( LOH ) at the retinoblastoma ( RB ) locus by Southern blot analysis or restriction fragment length polymorphism .
	manualset3
137083	5	407572	13	NULL	NULL	0	NULL	retinoblastoma ( RB ) locus	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of osteosarcoma cell lines or frozen tissue have detected loss of heterozygosity ( LOH ) at the retinoblastoma ( RB ) locus by Southern blot analysis or restriction fragment length polymorphism .
	manualset3
137084	6	407572	13	NULL	NULL	0	NULL	Southern blot analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of osteosarcoma cell lines or frozen tissue have detected loss of heterozygosity ( LOH ) at the retinoblastoma ( RB ) locus by Southern blot analysis or restriction fragment length polymorphism .
	manualset3
137085	7	407572	13	NULL	NULL	0	NULL	restriction fragment length polymorphism	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of osteosarcoma cell lines or frozen tissue have detected loss of heterozygosity ( LOH ) at the retinoblastoma ( RB ) locus by Southern blot analysis or restriction fragment length polymorphism .
	manualset3
137086	1	407573	13	NULL	NULL	0	NULL	Studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of privileged sites and islet transplantation .
	manualset3
137087	2	407573	13	NULL	NULL	0	NULL	privileged sites	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of privileged sites and islet transplantation .
	manualset3
137088	3	407573	13	NULL	NULL	0	NULL	islet transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of privileged sites and islet transplantation .
	manualset3
137089	1	407574	13	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of the effects of gemcitabine on ribonucleotide reduction in HL-60 cells revealed that dGTP pools , but not dCTP pools , were reduced by a 3-hour exposure to 40 nmol/L gemcitabine ( the concentration that causes 50 % lethality ) .
	manualset3
137090	2	407574	13	NULL	NULL	NULL	NULL	effects 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Studies of the effects of gemcitabine on ribonucleotide reduction in HL-60 cells revealed that dGTP pools , but not dCTP pools , were reduced by a 3-hour exposure to 40 nmol/L gemcitabine ( the concentration that causes 50 % lethality ) .
	manualset3
137091	3	407574	13	NULL	NULL	NULL	NULL	gemcitabine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Studies of the effects of gemcitabine on ribonucleotide reduction in HL-60 cells revealed that dGTP pools , but not dCTP pools , were reduced by a 3-hour exposure to 40 nmol/L gemcitabine ( the concentration that causes 50 % lethality ) .
	manualset3
137092	4	407574	13	NULL	NULL	0	NULL	ribonucleotide reduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of the effects of gemcitabine on ribonucleotide reduction in HL-60 cells revealed that dGTP pools , but not dCTP pools , were reduced by a 3-hour exposure to 40 nmol/L gemcitabine ( the concentration that causes 50 % lethality ) .
	manualset3
137093	5	407574	13	NULL	NULL	0	NULL	HL-60 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of the effects of gemcitabine on ribonucleotide reduction in HL-60 cells revealed that dGTP pools , but not dCTP pools , were reduced by a 3-hour exposure to 40 nmol/L gemcitabine ( the concentration that causes 50 % lethality ) .
	manualset3
137094	6	407574	13	NULL	NULL	0	NULL	dGTP pools	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of the effects of gemcitabine on ribonucleotide reduction in HL-60 cells revealed that dGTP pools , but not dCTP pools , were reduced by a 3-hour exposure to 40 nmol/L gemcitabine ( the concentration that causes 50 % lethality ) .
	manualset3
137095	7	407574	13	NULL	NULL	0	NULL	dCTP pools 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of the effects of gemcitabine on ribonucleotide reduction in HL-60 cells revealed that dGTP pools , but not dCTP pools , were reduced by a 3-hour exposure to 40 nmol/L gemcitabine ( the concentration that causes 50 % lethality ) .
	manualset3
137096	8	407574	13	NULL	NULL	0	NULL	3-hour	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of the effects of gemcitabine on ribonucleotide reduction in HL-60 cells revealed that dGTP pools , but not dCTP pools , were reduced by a 3-hour exposure to 40 nmol/L gemcitabine ( the concentration that causes 50 % lethality ) .
	manualset3
137097	9	407574	13	NULL	NULL	0	NULL	exposure 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of the effects of gemcitabine on ribonucleotide reduction in HL-60 cells revealed that dGTP pools , but not dCTP pools , were reduced by a 3-hour exposure to 40 nmol/L gemcitabine ( the concentration that causes 50 % lethality ) .
	manualset3
137098	10	407574	13	NULL	NULL	0	NULL	40 nmol/L 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of the effects of gemcitabine on ribonucleotide reduction in HL-60 cells revealed that dGTP pools , but not dCTP pools , were reduced by a 3-hour exposure to 40 nmol/L gemcitabine ( the concentration that causes 50 % lethality ) .
	manualset3
137099	11	407574	13	NULL	NULL	0	NULL	gemcitabine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of the effects of gemcitabine on ribonucleotide reduction in HL-60 cells revealed that dGTP pools , but not dCTP pools , were reduced by a 3-hour exposure to 40 nmol/L gemcitabine ( the concentration that causes 50 % lethality ) .
	manualset3
137100	12	407574	13	NULL	NULL	0	NULL	 concentration 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of the effects of gemcitabine on ribonucleotide reduction in HL-60 cells revealed that dGTP pools , but not dCTP pools , were reduced by a 3-hour exposure to 40 nmol/L gemcitabine ( the concentration that causes 50 % lethality ) .
	manualset3
137101	13	407574	13	NULL	NULL	0	NULL	50 % lethality 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of the effects of gemcitabine on ribonucleotide reduction in HL-60 cells revealed that dGTP pools , but not dCTP pools , were reduced by a 3-hour exposure to 40 nmol/L gemcitabine ( the concentration that causes 50 % lethality ) .
	manualset3
137102	1	407575	13	NULL	NULL	0	NULL	positive correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A positive correlation was found between TH-immunohistochemical intensity and the presence of GCHI mRNA .
	manualset3
137103	2	407575	13	NULL	NULL	0	NULL	TH-immunohistochemical intensity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A positive correlation was found between TH-immunohistochemical intensity and the presence of GCHI mRNA .
	manualset3
137104	3	407575	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A positive correlation was found between TH-immunohistochemical intensity and the presence of GCHI mRNA .
	manualset3
137105	4	407575	13	NULL	NULL	0	NULL	GCHI mRNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A positive correlation was found between TH-immunohistochemical intensity and the presence of GCHI mRNA .
	manualset3
137106	1	407576	13	NULL	NULL	0	NULL	Studies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of the lungs in diabetes mellitus .
	manualset3
137107	2	407576	13	NULL	NULL	0	NULL	lungs 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of the lungs in diabetes mellitus .
	manualset3
137108	3	407576	13	NULL	NULL	0	NULL	diabetes mellitus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of the lungs in diabetes mellitus .
	manualset3
137109	1	407577	13	NULL	NULL	0	NULL	Studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of the spore content of air in dwellings .
	manualset3
137110	2	407577	13	NULL	NULL	0	NULL	spore content	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of the spore content of air in dwellings .
	manualset3
137111	3	407577	13	NULL	NULL	0	NULL	air	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of the spore content of air in dwellings .
	manualset3
137112	4	407577	13	NULL	NULL	0	NULL	dwellings 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of the spore content of air in dwellings .
	manualset3
137113	1	407578	13	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on a possible molecular basis for the structure of mitochondrial cristae .
	manualset3
137114	2	407578	13	NULL	NULL	0	NULL	molecular basis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on a possible molecular basis for the structure of mitochondrial cristae .
	manualset3
137115	3	407578	13	NULL	NULL	0	NULL	structure 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on a possible molecular basis for the structure of mitochondrial cristae .
	manualset3
137116	4	407578	13	NULL	NULL	0	NULL	mitochondrial cristae	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on a possible molecular basis for the structure of mitochondrial cristae .
	manualset3
137117	1	407579	13	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on gene function by gene disruption and complementation indicated that scrX may play a positive regulation role in spore formation of Streptomyces coelicolor .
	manualset3
137118	2	407579	13	NULL	NULL	0	NULL	gene function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on gene function by gene disruption and complementation indicated that scrX may play a positive regulation role in spore formation of Streptomyces coelicolor .
	manualset3
137119	3	407579	13	NULL	NULL	0	NULL	gene disruption	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on gene function by gene disruption and complementation indicated that scrX may play a positive regulation role in spore formation of Streptomyces coelicolor .
	manualset3
137120	4	407579	13	NULL	NULL	0	NULL	complementation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on gene function by gene disruption and complementation indicated that scrX may play a positive regulation role in spore formation of Streptomyces coelicolor .
	manualset3
137121	5	407579	13	NULL	NULL	0	NULL	scrX 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on gene function by gene disruption and complementation indicated that scrX may play a positive regulation role in spore formation of Streptomyces coelicolor .
	manualset3
137122	6	407579	13	NULL	NULL	NULL	NULL	positive regulation role	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Studies on gene function by gene disruption and complementation indicated that scrX may play a positive regulation role in spore formation of Streptomyces coelicolor .
	manualset3
137123	7	407579	13	NULL	NULL	0	NULL	spore formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on gene function by gene disruption and complementation indicated that scrX may play a positive regulation role in spore formation of Streptomyces coelicolor .
	manualset3
137124	8	407579	13	NULL	NULL	0	NULL	Streptomyces coelicolor	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on gene function by gene disruption and complementation indicated that scrX may play a positive regulation role in spore formation of Streptomyces coelicolor .
	manualset3
137128	1	407580	13	NULL	NULL	0	NULL	Studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on localization of enzyme activity at the ultrastructural level in unfixed specimens , be it fresh or frozen , are reviewed here .
	manualset3
137129	2	407580	13	NULL	NULL	0	NULL	localization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on localization of enzyme activity at the ultrastructural level in unfixed specimens , be it fresh or frozen , are reviewed here .
	manualset3
137130	3	407580	13	NULL	NULL	0	NULL	enzyme activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on localization of enzyme activity at the ultrastructural level in unfixed specimens , be it fresh or frozen , are reviewed here .
	manualset3
137140	4	407580	13	NULL	NULL	0	NULL	ultrastructural level	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on localization of enzyme activity at the ultrastructural level in unfixed specimens , be it fresh or frozen , are reviewed here .
	manualset3
137141	5	407580	13	NULL	NULL	0	NULL	specimens 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on localization of enzyme activity at the ultrastructural level in unfixed specimens , be it fresh or frozen , are reviewed here .
	manualset3
137142	1	407581	13	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on maturity in newborn infants .
	manualset3
137143	2	407581	13	NULL	NULL	0	NULL	maturity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on maturity in newborn infants .
	manualset3
137144	3	407581	13	NULL	NULL	0	NULL	newborn infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on maturity in newborn infants .
	manualset3
137145	1	407582	13	NULL	NULL	0	NULL	Studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on synthetic antimalarial drugs ; the absorption , distribution and excretion of paludrine in experimental animals .
	manualset3
137146	2	407582	13	NULL	NULL	0	NULL	synthetic antimalarial drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on synthetic antimalarial drugs ; the absorption , distribution and excretion of paludrine in experimental animals .
	manualset3
137147	3	407582	13	NULL	NULL	0	NULL	absorption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on synthetic antimalarial drugs ; the absorption , distribution and excretion of paludrine in experimental animals .
	manualset3
137148	4	407582	13	NULL	NULL	0	NULL	distribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on synthetic antimalarial drugs ; the absorption , distribution and excretion of paludrine in experimental animals .
	manualset3
137149	5	407582	13	NULL	NULL	0	NULL	excretion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on synthetic antimalarial drugs ; the absorption , distribution and excretion of paludrine in experimental animals .
	manualset3
137150	6	407582	13	NULL	NULL	0	NULL	paludrine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on synthetic antimalarial drugs ; the absorption , distribution and excretion of paludrine in experimental animals .
	manualset3
137151	7	407582	13	NULL	NULL	0	NULL	experimental animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on synthetic antimalarial drugs ; the absorption , distribution and excretion of paludrine in experimental animals .
	manualset3
137152	1	407583	13	NULL	NULL	0	NULL	Studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on the optimum conditions of extraction of silicon species from plants with water .
	manualset3
137170	2	407583	13	NULL	NULL	0	NULL	optimum conditions 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on the optimum conditions of extraction of silicon species from plants with water .
	manualset3
137172	3	407583	13	NULL	NULL	0	NULL	extraction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on the optimum conditions of extraction of silicon species from plants with water .
	manualset3
137173	4	407583	13	NULL	NULL	0	NULL	silicon species 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on the optimum conditions of extraction of silicon species from plants with water .
	manualset3
137174	5	407583	13	NULL	NULL	0	NULL	plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on the optimum conditions of extraction of silicon species from plants with water .
	manualset3
137175	6	407583	13	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on the optimum conditions of extraction of silicon species from plants with water .
	manualset3
137180	1	407584	13	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on the ribothymidine content of specific rat and human tRNAs : a postulated role for 5-methyl cytosine in the regulation of ribothymidine biosynthesis .
	manualset3
137184	2	407584	13	NULL	NULL	0	NULL	ribothymidine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on the ribothymidine content of specific rat and human tRNAs : a postulated role for 5-methyl cytosine in the regulation of ribothymidine biosynthesis .
	manualset3
137188	3	407584	13	NULL	NULL	0	NULL	content	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on the ribothymidine content of specific rat and human tRNAs : a postulated role for 5-methyl cytosine in the regulation of ribothymidine biosynthesis .
	manualset3
137190	4	407584	13	NULL	NULL	0	NULL	rat tRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on the ribothymidine content of specific rat and human tRNAs : a postulated role for 5-methyl cytosine in the regulation of ribothymidine biosynthesis .
	manualset3
137191	5	407584	13	NULL	NULL	0	NULL	human tRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on the ribothymidine content of specific rat and human tRNAs : a postulated role for 5-methyl cytosine in the regulation of ribothymidine biosynthesis .
	manualset3
137237	6	407584	13	NULL	NULL	0	NULL	role 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on the ribothymidine content of specific rat and human tRNAs : a postulated role for 5-methyl cytosine in the regulation of ribothymidine biosynthesis .
	manualset3
137238	7	407584	13	NULL	NULL	0	NULL	5-methyl cytosine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on the ribothymidine content of specific rat and human tRNAs : a postulated role for 5-methyl cytosine in the regulation of ribothymidine biosynthesis .
	manualset3
137239	8	407584	13	NULL	NULL	0	NULL	regulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on the ribothymidine content of specific rat and human tRNAs : a postulated role for 5-methyl cytosine in the regulation of ribothymidine biosynthesis .
	manualset3
137240	9	407584	13	NULL	NULL	0	NULL	ribothymidine biosynthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on the ribothymidine content of specific rat and human tRNAs : a postulated role for 5-methyl cytosine in the regulation of ribothymidine biosynthesis .
	manualset3
137283	1	407585	13	NULL	NULL	0	NULL	Studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies suggest that the therapeutic effects of ARBs may reflect this unopposed activation of the AT2R in addition to the inhibition of the AT1R .
	manualset3
137284	2	407585	13	NULL	NULL	0	NULL	therapeutic effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies suggest that the therapeutic effects of ARBs may reflect this unopposed activation of the AT2R in addition to the inhibition of the AT1R .
	manualset3
137293	3	407585	13	NULL	NULL	0	NULL	ARBs 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies suggest that the therapeutic effects of ARBs may reflect this unopposed activation of the AT2R in addition to the inhibition of the AT1R .
	manualset3
137294	4	407585	13	NULL	NULL	0	NULL	activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies suggest that the therapeutic effects of ARBs may reflect this unopposed activation of the AT2R in addition to the inhibition of the AT1R .
	manualset3
137295	5	407585	13	NULL	NULL	0	NULL	AT2R	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies suggest that the therapeutic effects of ARBs may reflect this unopposed activation of the AT2R in addition to the inhibition of the AT1R .
	manualset3
137296	6	407585	13	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies suggest that the therapeutic effects of ARBs may reflect this unopposed activation of the AT2R in addition to the inhibition of the AT1R .
	manualset3
137298	7	407585	13	NULL	NULL	0	NULL	inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies suggest that the therapeutic effects of ARBs may reflect this unopposed activation of the AT2R in addition to the inhibition of the AT1R .
	manualset3
137299	8	407585	13	NULL	NULL	0	NULL	AT1R	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies suggest that the therapeutic effects of ARBs may reflect this unopposed activation of the AT2R in addition to the inhibition of the AT1R .
	manualset3
137303	1	407586	13	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies using luciferase reporters carrying wild-type ( WT ) and mutant IL-6 3 ` UTR confirmed IL-6 as a target for miR-142-3p .
	manualset3
137304	2	407586	13	NULL	NULL	0	NULL	luciferase reporters 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies using luciferase reporters carrying wild-type ( WT ) and mutant IL-6 3 ` UTR confirmed IL-6 as a target for miR-142-3p .
	manualset3
137306	3	407586	13	NULL	NULL	0	NULL	wild-type ( WT ) IL-6 3 ` UTR	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies using luciferase reporters carrying wild-type ( WT ) and mutant IL-6 3 ` UTR confirmed IL-6 as a target for miR-142-3p .
	manualset3
137307	4	407586	13	NULL	NULL	0	NULL	mutant IL-6 3 ` UTR	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies using luciferase reporters carrying wild-type ( WT ) and mutant IL-6 3 ` UTR confirmed IL-6 as a target for miR-142-3p .
	manualset3
137310	5	407586	13	NULL	NULL	0	NULL	IL-6	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies using luciferase reporters carrying wild-type ( WT ) and mutant IL-6 3 ` UTR confirmed IL-6 as a target for miR-142-3p .
	manualset3
137311	6	407586	13	NULL	NULL	0	NULL	target 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies using luciferase reporters carrying wild-type ( WT ) and mutant IL-6 3 ` UTR confirmed IL-6 as a target for miR-142-3p .
	manualset3
137312	7	407586	13	NULL	NULL	0	NULL	 miR-142-3p	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies using luciferase reporters carrying wild-type ( WT ) and mutant IL-6 3 ` UTR confirmed IL-6 as a target for miR-142-3p .
	manualset3
137313	1	407587	13	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies using mouse models of cancer suggest that methods that integrate genetic analysis and genomic networks with knowledge of cancer biology can help to extend our understanding of heritable cancer susceptibility .
	manualset3
137314	2	407587	13	NULL	NULL	0	NULL	mouse models	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies using mouse models of cancer suggest that methods that integrate genetic analysis and genomic networks with knowledge of cancer biology can help to extend our understanding of heritable cancer susceptibility .
	manualset3
137315	3	407587	13	NULL	NULL	0	NULL	cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies using mouse models of cancer suggest that methods that integrate genetic analysis and genomic networks with knowledge of cancer biology can help to extend our understanding of heritable cancer susceptibility .
	manualset3
137316	4	407587	13	NULL	NULL	0	NULL	methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies using mouse models of cancer suggest that methods that integrate genetic analysis and genomic networks with knowledge of cancer biology can help to extend our understanding of heritable cancer susceptibility .
	manualset3
137317	5	407587	13	NULL	NULL	0	NULL	genetic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies using mouse models of cancer suggest that methods that integrate genetic analysis and genomic networks with knowledge of cancer biology can help to extend our understanding of heritable cancer susceptibility .
	manualset3
137318	6	407587	13	NULL	NULL	0	NULL	genomic networks	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies using mouse models of cancer suggest that methods that integrate genetic analysis and genomic networks with knowledge of cancer biology can help to extend our understanding of heritable cancer susceptibility .
	manualset3
137319	7	407587	13	NULL	NULL	0	NULL	knowledge	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies using mouse models of cancer suggest that methods that integrate genetic analysis and genomic networks with knowledge of cancer biology can help to extend our understanding of heritable cancer susceptibility .
	manualset3
137320	8	407587	13	NULL	NULL	0	NULL	cancer biology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies using mouse models of cancer suggest that methods that integrate genetic analysis and genomic networks with knowledge of cancer biology can help to extend our understanding of heritable cancer susceptibility .
	manualset3
137321	9	407587	13	NULL	NULL	0	NULL	understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies using mouse models of cancer suggest that methods that integrate genetic analysis and genomic networks with knowledge of cancer biology can help to extend our understanding of heritable cancer susceptibility .
	manualset3
137322	10	407587	13	NULL	NULL	0	NULL	heritable cancer susceptibility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies using mouse models of cancer suggest that methods that integrate genetic analysis and genomic networks with knowledge of cancer biology can help to extend our understanding of heritable cancer susceptibility .
	manualset3
137323	1	407588	13	NULL	NULL	0	NULL	Studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies using these assays have demonstrated that both MeIQx and PhIP are well absorbed and extensively metabolised following ingestion of amine-containing beef by humans .
	manualset3
137324	2	407588	13	NULL	NULL	0	NULL	assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies using these assays have demonstrated that both MeIQx and PhIP are well absorbed and extensively metabolised following ingestion of amine-containing beef by humans .
	manualset3
137325	3	407588	13	NULL	NULL	0	NULL	MeIQx	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies using these assays have demonstrated that both MeIQx and PhIP are well absorbed and extensively metabolised following ingestion of amine-containing beef by humans .
	manualset3
137326	4	407588	13	NULL	NULL	0	NULL	PhIP 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies using these assays have demonstrated that both MeIQx and PhIP are well absorbed and extensively metabolised following ingestion of amine-containing beef by humans .
	manualset3
137327	5	407588	13	NULL	NULL	0	NULL	ingestion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies using these assays have demonstrated that both MeIQx and PhIP are well absorbed and extensively metabolised following ingestion of amine-containing beef by humans .
	manualset3
137328	6	407588	13	NULL	NULL	0	NULL	beef 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies using these assays have demonstrated that both MeIQx and PhIP are well absorbed and extensively metabolised following ingestion of amine-containing beef by humans .
	manualset3
137329	7	407588	13	NULL	NULL	0	NULL	humans	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies using these assays have demonstrated that both MeIQx and PhIP are well absorbed and extensively metabolised following ingestion of amine-containing beef by humans .
	manualset3
137330	1	407589	13	NULL	NULL	0	NULL	Studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies were done to investigate the potential inheritance of the idiotype in families ; in three of four families the idiotype was inherited in an apparent autosomal dominant pattern .
	manualset3
137331	2	407589	13	NULL	NULL	0	NULL	inheritance 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies were done to investigate the potential inheritance of the idiotype in families ; in three of four families the idiotype was inherited in an apparent autosomal dominant pattern .
	manualset3
137333	3	407589	13	NULL	NULL	0	NULL	idiotype 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies were done to investigate the potential inheritance of the idiotype in families ; in three of four families the idiotype was inherited in an apparent autosomal dominant pattern .
	manualset3
137336	4	407589	13	NULL	NULL	0	NULL	families	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies were done to investigate the potential inheritance of the idiotype in families ; in three of four families the idiotype was inherited in an apparent autosomal dominant pattern .
	manualset3
137339	5	407589	13	NULL	NULL	0	NULL	three of four families 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies were done to investigate the potential inheritance of the idiotype in families ; in three of four families the idiotype was inherited in an apparent autosomal dominant pattern .
	manualset3
137341	6	407589	13	NULL	NULL	0	NULL	idiotype	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies were done to investigate the potential inheritance of the idiotype in families ; in three of four families the idiotype was inherited in an apparent autosomal dominant pattern .
	manualset3
137342	7	407589	13	NULL	NULL	0	NULL	autosomal dominant pattern 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies were done to investigate the potential inheritance of the idiotype in families ; in three of four families the idiotype was inherited in an apparent autosomal dominant pattern .
	manualset3
137345	1	407590	13	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies with seismic waves , ocean acoustics , and laboratory ultrasound have confirmed them .
	manualset3
137346	2	407590	13	NULL	NULL	0	NULL	seismic waves	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies with seismic waves , ocean acoustics , and laboratory ultrasound have confirmed them .
	manualset3
137347	3	407590	13	NULL	NULL	0	NULL	ocean acoustics 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies with seismic waves , ocean acoustics , and laboratory ultrasound have confirmed them .
	manualset3
137348	4	407590	13	NULL	NULL	0	NULL	laboratory ultrasound	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies with seismic waves , ocean acoustics , and laboratory ultrasound have confirmed them .
	manualset3
137350	1	407591	13	NULL	NULL	0	NULL	Study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Study of casualty patients at an urban hospital .
	manualset3
137351	2	407591	13	NULL	NULL	0	NULL	casualty patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Study of casualty patients at an urban hospital .
	manualset3
137353	3	407591	13	NULL	NULL	0	NULL	urban hospital	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Study of casualty patients at an urban hospital .
	manualset3
137355	1	407592	13	NULL	NULL	0	NULL	Study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Study of nitrogenase activity in the mycorrhizal rhizosphere of pine and oak .
	manualset3
137358	2	407592	13	NULL	NULL	0	NULL	nitrogenase activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Study of nitrogenase activity in the mycorrhizal rhizosphere of pine and oak .
	manualset3
137362	3	407592	13	NULL	NULL	0	NULL	mycorrhizal rhizosphere	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Study of nitrogenase activity in the mycorrhizal rhizosphere of pine and oak .
	manualset3
137363	4	407592	13	NULL	NULL	0	NULL	pine	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Study of nitrogenase activity in the mycorrhizal rhizosphere of pine and oak .
	manualset3
137364	5	407592	13	NULL	NULL	0	NULL	oak	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Study of nitrogenase activity in the mycorrhizal rhizosphere of pine and oak .
	manualset3
137365	1	407593	13	NULL	NULL	0	NULL	positive reaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A positive reaction was found in various tissue cells , including nerve cells , myelin sheaths , glia cells , hepatocytes , cells of the alveolar and bronchial wall , epithelial cells of the distal part of the renal tubules , and so forth .
	manualset3
137366	2	407593	13	NULL	NULL	0	NULL	tissue cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A positive reaction was found in various tissue cells , including nerve cells , myelin sheaths , glia cells , hepatocytes , cells of the alveolar and bronchial wall , epithelial cells of the distal part of the renal tubules , and so forth .
	manualset3
137367	3	407593	13	NULL	NULL	0	NULL	nerve cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A positive reaction was found in various tissue cells , including nerve cells , myelin sheaths , glia cells , hepatocytes , cells of the alveolar and bronchial wall , epithelial cells of the distal part of the renal tubules , and so forth .
	manualset3
137368	4	407593	13	NULL	NULL	0	NULL	myelin sheaths	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A positive reaction was found in various tissue cells , including nerve cells , myelin sheaths , glia cells , hepatocytes , cells of the alveolar and bronchial wall , epithelial cells of the distal part of the renal tubules , and so forth .
	manualset3
137369	5	407593	13	NULL	NULL	0	NULL	glia cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A positive reaction was found in various tissue cells , including nerve cells , myelin sheaths , glia cells , hepatocytes , cells of the alveolar and bronchial wall , epithelial cells of the distal part of the renal tubules , and so forth .
	manualset3
137370	6	407593	13	NULL	NULL	0	NULL	hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A positive reaction was found in various tissue cells , including nerve cells , myelin sheaths , glia cells , hepatocytes , cells of the alveolar and bronchial wall , epithelial cells of the distal part of the renal tubules , and so forth .
	manualset3
137371	7	407593	13	NULL	NULL	NULL	NULL	cells of the alveolar wall	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A positive reaction was found in various tissue cells , including nerve cells , myelin sheaths , glia cells , hepatocytes , cells of the alveolar and bronchial wall , epithelial cells of the distal part of the renal tubules , and so forth .
	manualset3
137372	8	407593	13	NULL	NULL	0	NULL	cells of the bronchial wall	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A positive reaction was found in various tissue cells , including nerve cells , myelin sheaths , glia cells , hepatocytes , cells of the alveolar and bronchial wall , epithelial cells of the distal part of the renal tubules , and so forth .
	manualset3
137373	9	407593	13	NULL	NULL	0	NULL	epithelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A positive reaction was found in various tissue cells , including nerve cells , myelin sheaths , glia cells , hepatocytes , cells of the alveolar and bronchial wall , epithelial cells of the distal part of the renal tubules , and so forth .
	manualset3
137374	10	407593	13	NULL	NULL	0	NULL	distal part of the renal tubules	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A positive reaction was found in various tissue cells , including nerve cells , myelin sheaths , glia cells , hepatocytes , cells of the alveolar and bronchial wall , epithelial cells of the distal part of the renal tubules , and so forth .
	manualset3
137375	1	407594	13	NULL	NULL	0	NULL	Study measures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Study measures assessing skin picking severity and impact , anxiety , depression , and quality of life were given at baseline and weeks 2 , 4 , 6 , 10 , 14 , and 18 .
	manualset3
137376	2	407594	13	NULL	NULL	0	NULL	skin picking severity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Study measures assessing skin picking severity and impact , anxiety , depression , and quality of life were given at baseline and weeks 2 , 4 , 6 , 10 , 14 , and 18 .
	manualset3
137377	3	407594	13	NULL	NULL	0	NULL	impact 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Study measures assessing skin picking severity and impact , anxiety , depression , and quality of life were given at baseline and weeks 2 , 4 , 6 , 10 , 14 , and 18 .
	manualset3
137378	4	407594	13	NULL	NULL	0	NULL	anxiety	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Study measures assessing skin picking severity and impact , anxiety , depression , and quality of life were given at baseline and weeks 2 , 4 , 6 , 10 , 14 , and 18 .
	manualset3
137379	5	407594	13	NULL	NULL	0	NULL	depression 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Study measures assessing skin picking severity and impact , anxiety , depression , and quality of life were given at baseline and weeks 2 , 4 , 6 , 10 , 14 , and 18 .
	manualset3
137380	6	407594	13	NULL	NULL	0	NULL	quality of life	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Study measures assessing skin picking severity and impact , anxiety , depression , and quality of life were given at baseline and weeks 2 , 4 , 6 , 10 , 14 , and 18 .
	manualset3
137381	7	407594	13	NULL	NULL	0	NULL	baseline 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Study measures assessing skin picking severity and impact , anxiety , depression , and quality of life were given at baseline and weeks 2 , 4 , 6 , 10 , 14 , and 18 .
	manualset3
137382	8	407594	13	NULL	NULL	NULL	NULL	week 2	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Study measures assessing skin picking severity and impact , anxiety , depression , and quality of life were given at baseline and weeks 2 , 4 , 6 , 10 , 14 , and 18 .
	manualset3
137383	9	407594	13	NULL	NULL	0	NULL	week 4	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Study measures assessing skin picking severity and impact , anxiety , depression , and quality of life were given at baseline and weeks 2 , 4 , 6 , 10 , 14 , and 18 .
	manualset3
137384	10	407594	13	NULL	NULL	0	NULL	week 6	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Study measures assessing skin picking severity and impact , anxiety , depression , and quality of life were given at baseline and weeks 2 , 4 , 6 , 10 , 14 , and 18 .
	manualset3
137385	11	407594	13	NULL	NULL	NULL	NULL	week 10	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Study measures assessing skin picking severity and impact , anxiety , depression , and quality of life were given at baseline and weeks 2 , 4 , 6 , 10 , 14 , and 18 .
	manualset3
137386	12	407594	13	NULL	NULL	0	NULL	week 14	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Study measures assessing skin picking severity and impact , anxiety , depression , and quality of life were given at baseline and weeks 2 , 4 , 6 , 10 , 14 , and 18 .
	manualset3
137387	13	407594	13	NULL	NULL	0	NULL	week 18	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Study measures assessing skin picking severity and impact , anxiety , depression , and quality of life were given at baseline and weeks 2 , 4 , 6 , 10 , 14 , and 18 .
	manualset3
137388	1	407595	13	NULL	NULL	0	NULL	Avicenna 's Canon of Medicine	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Studying the Avicenna 's Canon of Medicine , provides noteworthy information on the subjects related to urology .
	manualset3
137389	2	407595	13	NULL	NULL	NULL	NULL	information	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Studying the Avicenna 's Canon of Medicine , provides noteworthy information on the subjects related to urology .
	manualset3
137390	3	407595	13	NULL	NULL	0	NULL	subjects 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studying the Avicenna 's Canon of Medicine , provides noteworthy information on the subjects related to urology .
	manualset3
137391	4	407595	13	NULL	NULL	0	NULL	urology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Studying the Avicenna 's Canon of Medicine , provides noteworthy information on the subjects related to urology .
	manualset3
137405	1	407596	13	NULL	NULL	0	NULL	HT-29 colon cancer cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Studying the HT-29 colon cancer cell line as a model , we found that Cox-2 mRNA and protein levels were activated over 10-fold by the inflammatory cytokine tumor necrosis factor ( TNF ) - alpha .
	manualset3
137406	2	407596	13	NULL	NULL	0	NULL	model	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Studying the HT-29 colon cancer cell line as a model , we found that Cox-2 mRNA and protein levels were activated over 10-fold by the inflammatory cytokine tumor necrosis factor ( TNF ) - alpha .
	manualset3
137407	3	407596	13	NULL	NULL	0	NULL	Cox-2 mRNA levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Studying the HT-29 colon cancer cell line as a model , we found that Cox-2 mRNA and protein levels were activated over 10-fold by the inflammatory cytokine tumor necrosis factor ( TNF ) - alpha .
	manualset3
137408	4	407596	13	NULL	NULL	0	NULL	Cox-2 protein levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Studying the HT-29 colon cancer cell line as a model , we found that Cox-2 mRNA and protein levels were activated over 10-fold by the inflammatory cytokine tumor necrosis factor ( TNF ) - alpha .
	manualset3
137409	5	407596	13	NULL	NULL	0	NULL	10-fold 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Studying the HT-29 colon cancer cell line as a model , we found that Cox-2 mRNA and protein levels were activated over 10-fold by the inflammatory cytokine tumor necrosis factor ( TNF ) - alpha .
	manualset3
137411	6	407596	13	NULL	NULL	0	NULL	inflammatory cytokine tumor necrosis factor ( TNF ) - alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Studying the HT-29 colon cancer cell line as a model , we found that Cox-2 mRNA and protein levels were activated over 10-fold by the inflammatory cytokine tumor necrosis factor ( TNF ) - alpha .
	manualset3
137421	1	407597	13	NULL	NULL	0	NULL	dynamics	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studying the dynamics of age-related variations in the test parameters will contribute to the understanding of pathogenetic mechanisms and development of new methods for pharmacological correction of postnatal changes in CNS after hypoxia during early ontogeny .
	manualset3
137423	2	407597	13	NULL	NULL	0	NULL	age-related variations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studying the dynamics of age-related variations in the test parameters will contribute to the understanding of pathogenetic mechanisms and development of new methods for pharmacological correction of postnatal changes in CNS after hypoxia during early ontogeny .
	manualset3
137424	3	407597	13	NULL	NULL	0	NULL	test parameters 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studying the dynamics of age-related variations in the test parameters will contribute to the understanding of pathogenetic mechanisms and development of new methods for pharmacological correction of postnatal changes in CNS after hypoxia during early ontogeny .
	manualset3
137426	4	407597	13	NULL	NULL	0	NULL	understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studying the dynamics of age-related variations in the test parameters will contribute to the understanding of pathogenetic mechanisms and development of new methods for pharmacological correction of postnatal changes in CNS after hypoxia during early ontogeny .
	manualset3
137428	5	407597	13	NULL	NULL	0	NULL	 pathogenetic mechanisms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studying the dynamics of age-related variations in the test parameters will contribute to the understanding of pathogenetic mechanisms and development of new methods for pharmacological correction of postnatal changes in CNS after hypoxia during early ontogeny .
	manualset3
137429	6	407597	13	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Studying the dynamics of age-related variations in the test parameters will contribute to the understanding of pathogenetic mechanisms and development of new methods for pharmacological correction of postnatal changes in CNS after hypoxia during early ontogeny .
	manualset3
137431	7	407597	13	NULL	NULL	0	NULL	new methods	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Studying the dynamics of age-related variations in the test parameters will contribute to the understanding of pathogenetic mechanisms and development of new methods for pharmacological correction of postnatal changes in CNS after hypoxia during early ontogeny .
	manualset3
137432	8	407597	13	NULL	NULL	0	NULL	pharmacological correction 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Studying the dynamics of age-related variations in the test parameters will contribute to the understanding of pathogenetic mechanisms and development of new methods for pharmacological correction of postnatal changes in CNS after hypoxia during early ontogeny .
	manualset3
137433	9	407597	13	NULL	NULL	0	NULL	postnatal changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studying the dynamics of age-related variations in the test parameters will contribute to the understanding of pathogenetic mechanisms and development of new methods for pharmacological correction of postnatal changes in CNS after hypoxia during early ontogeny .
	manualset3
137434	10	407597	13	NULL	NULL	0	NULL	CNS	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Studying the dynamics of age-related variations in the test parameters will contribute to the understanding of pathogenetic mechanisms and development of new methods for pharmacological correction of postnatal changes in CNS after hypoxia during early ontogeny .
	manualset3
137436	11	407597	13	NULL	NULL	0	NULL	hypoxia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Studying the dynamics of age-related variations in the test parameters will contribute to the understanding of pathogenetic mechanisms and development of new methods for pharmacological correction of postnatal changes in CNS after hypoxia during early ontogeny .
	manualset3
137439	12	407597	13	NULL	NULL	0	NULL	ontogeny	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studying the dynamics of age-related variations in the test parameters will contribute to the understanding of pathogenetic mechanisms and development of new methods for pharmacological correction of postnatal changes in CNS after hypoxia during early ontogeny .
	manualset3
137461	1	407598	13	NULL	NULL	0	NULL	liquid gate effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Studying the liquid gate effect and ionic concentration dependence of strepavidin sensing indicates that electrostatic interaction is the dominant mechanism for sensing response .
	manualset3
137462	2	407598	13	NULL	NULL	0	NULL	ionic concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Studying the liquid gate effect and ionic concentration dependence of strepavidin sensing indicates that electrostatic interaction is the dominant mechanism for sensing response .
	manualset3
137464	3	407598	13	NULL	NULL	0	NULL	dependence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Studying the liquid gate effect and ionic concentration dependence of strepavidin sensing indicates that electrostatic interaction is the dominant mechanism for sensing response .
	manualset3
137479	4	407598	13	NULL	NULL	0	NULL	strepavidin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Studying the liquid gate effect and ionic concentration dependence of strepavidin sensing indicates that electrostatic interaction is the dominant mechanism for sensing response .
	manualset3
137481	5	407598	13	NULL	NULL	0	NULL	electrostatic interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studying the liquid gate effect and ionic concentration dependence of strepavidin sensing indicates that electrostatic interaction is the dominant mechanism for sensing response .
	manualset3
137483	6	407598	13	NULL	NULL	0	NULL	mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studying the liquid gate effect and ionic concentration dependence of strepavidin sensing indicates that electrostatic interaction is the dominant mechanism for sensing response .
	manualset3
137484	7	407598	13	NULL	NULL	0	NULL	response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studying the liquid gate effect and ionic concentration dependence of strepavidin sensing indicates that electrostatic interaction is the dominant mechanism for sensing response .
	manualset3
137488	1	407599	13	NULL	NULL	0	NULL	Subacute care 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Subacute care and other long-term care facilities often present unique challenges to pain management .
	manualset3
137490	2	407599	13	NULL	NULL	0	NULL	long-term care facilities	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Subacute care and other long-term care facilities often present unique challenges to pain management .
	manualset3
137491	3	407599	13	NULL	NULL	0	NULL	challenges 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subacute care and other long-term care facilities often present unique challenges to pain management .
	manualset3
137493	4	407599	13	NULL	NULL	0	NULL	pain management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Subacute care and other long-term care facilities often present unique challenges to pain management .
	manualset3
137498	1	407600	13	NULL	NULL	0	NULL	Subacute infantile mountain sickness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subacute infantile mountain sickness is a condition seen predominantly in Han Chinese infants living in Tibet , although it has been described in other high altitude communities as well .
	manualset3
137499	2	407600	13	NULL	NULL	0	NULL	condition 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subacute infantile mountain sickness is a condition seen predominantly in Han Chinese infants living in Tibet , although it has been described in other high altitude communities as well .
	manualset3
137500	3	407600	13	NULL	NULL	0	NULL	Han Chinese infants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subacute infantile mountain sickness is a condition seen predominantly in Han Chinese infants living in Tibet , although it has been described in other high altitude communities as well .
	manualset3
137502	4	407600	13	NULL	NULL	0	NULL	Tibet 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Subacute infantile mountain sickness is a condition seen predominantly in Han Chinese infants living in Tibet , although it has been described in other high altitude communities as well .
	manualset3
137503	5	407600	13	NULL	NULL	0	NULL	high altitude communities	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subacute infantile mountain sickness is a condition seen predominantly in Han Chinese infants living in Tibet , although it has been described in other high altitude communities as well .
	manualset3
137508	1	407601	13	NULL	NULL	0	NULL	Subarachnoid hemorrhage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subarachnoid hemorrhage associated with epidemic hemorrhagic fever : a rare case report .
	manualset3
137510	2	407601	13	NULL	NULL	0	NULL	epidemic hemorrhagic fever	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Subarachnoid hemorrhage associated with epidemic hemorrhagic fever : a rare case report .
	manualset3
137511	3	407601	13	NULL	NULL	0	NULL	case report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Subarachnoid hemorrhage associated with epidemic hemorrhagic fever : a rare case report .
	manualset3
137515	1	407602	13	NULL	NULL	0	NULL	Subcellular N-cadherin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Subcellular N-cadherin was accumulated in bands at intercellular junctions between SCs and was clustered at axon-SC contact sites .
	manualset3
137516	2	407602	13	NULL	NULL	0	NULL	bands	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subcellular N-cadherin was accumulated in bands at intercellular junctions between SCs and was clustered at axon-SC contact sites .
	manualset3
137528	3	407602	13	NULL	NULL	0	NULL	intercellular junctions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Subcellular N-cadherin was accumulated in bands at intercellular junctions between SCs and was clustered at axon-SC contact sites .
	manualset3
137530	4	407602	13	NULL	NULL	0	NULL	SCs 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Subcellular N-cadherin was accumulated in bands at intercellular junctions between SCs and was clustered at axon-SC contact sites .
	manualset3
137532	5	407602	13	NULL	NULL	0	NULL	axon-SC contact sites	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Subcellular N-cadherin was accumulated in bands at intercellular junctions between SCs and was clustered at axon-SC contact sites .
	manualset3
137535	1	407603	13	NULL	NULL	0	NULL	Subclavian aneurysm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subclavian aneurysm producing the subclavian steal syndrome .
	manualset3
137536	2	407603	13	NULL	NULL	0	NULL	subclavian steal syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Subclavian aneurysm producing the subclavian steal syndrome .
	manualset3
137537	1	407604	13	NULL	NULL	0	NULL	Subclinical effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subclinical effects of T. gondii infection on lamb weight , litter size , total litter weight and ewe weight were also studied .
	manualset3
137538	2	407604	13	NULL	NULL	0	NULL	T. gondii infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subclinical effects of T. gondii infection on lamb weight , litter size , total litter weight and ewe weight were also studied .
	manualset3
137541	3	407604	13	NULL	NULL	0	NULL	lamb weight	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Subclinical effects of T. gondii infection on lamb weight , litter size , total litter weight and ewe weight were also studied .
	manualset3
137543	4	407604	13	NULL	NULL	0	NULL	litter size	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Subclinical effects of T. gondii infection on lamb weight , litter size , total litter weight and ewe weight were also studied .
	manualset3
137545	5	407604	13	NULL	NULL	0	NULL	total litter weight 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Subclinical effects of T. gondii infection on lamb weight , litter size , total litter weight and ewe weight were also studied .
	manualset3
137546	6	407604	13	NULL	NULL	0	NULL	ewe weight	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Subclinical effects of T. gondii infection on lamb weight , litter size , total litter weight and ewe weight were also studied .
	manualset3
138234	1	407605	13	NULL	NULL	0	NULL	Subclones of C3/23	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Subclones of C3/23 were used to show that the 3 ' flanking region was conserved in all strains examined in this study and was repeated many times in the genome .
	manualset3
138235	2	407605	13	NULL	NULL	0	NULL	3 ' flanking region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Subclones of C3/23 were used to show that the 3 ' flanking region was conserved in all strains examined in this study and was repeated many times in the genome .
	manualset3
138236	3	407605	13	NULL	NULL	0	NULL	strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Subclones of C3/23 were used to show that the 3 ' flanking region was conserved in all strains examined in this study and was repeated many times in the genome .
	manualset3
138237	4	407605	13	NULL	NULL	0	NULL	study	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subclones of C3/23 were used to show that the 3 ' flanking region was conserved in all strains examined in this study and was repeated many times in the genome .
	manualset3
138238	5	407605	13	NULL	NULL	0	NULL	genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Subclones of C3/23 were used to show that the 3 ' flanking region was conserved in all strains examined in this study and was repeated many times in the genome .
	manualset3
138239	1	407606	13	NULL	NULL	0	NULL	Subcutaneous emphysema 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subcutaneous emphysema and pneumomediastinum following shoulder arthroscopy with brachial plexus block : a case report and review of the literature .
	manualset3
138240	2	407606	13	NULL	NULL	0	NULL	pneumomediastinum 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subcutaneous emphysema and pneumomediastinum following shoulder arthroscopy with brachial plexus block : a case report and review of the literature .
	manualset3
138241	3	407606	13	NULL	NULL	0	NULL	shoulder arthroscopy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Subcutaneous emphysema and pneumomediastinum following shoulder arthroscopy with brachial plexus block : a case report and review of the literature .
	manualset3
138242	4	407606	13	NULL	NULL	0	NULL	brachial plexus block 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Subcutaneous emphysema and pneumomediastinum following shoulder arthroscopy with brachial plexus block : a case report and review of the literature .
	manualset3
138243	5	407606	13	NULL	NULL	0	NULL	case report 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Subcutaneous emphysema and pneumomediastinum following shoulder arthroscopy with brachial plexus block : a case report and review of the literature .
	manualset3
138244	6	407606	13	NULL	NULL	0	NULL	review	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subcutaneous emphysema and pneumomediastinum following shoulder arthroscopy with brachial plexus block : a case report and review of the literature .
	manualset3
138245	7	407606	13	NULL	NULL	0	NULL	literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Subcutaneous emphysema and pneumomediastinum following shoulder arthroscopy with brachial plexus block : a case report and review of the literature .
	manualset3
138246	1	407607	13	NULL	NULL	0	NULL	Subcutaneous infusions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Subcutaneous infusions of gammaglobulin are usually given at a slow rate .
	manualset3
138247	2	407607	13	NULL	NULL	0	NULL	gammaglobulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Subcutaneous infusions of gammaglobulin are usually given at a slow rate .
	manualset3
138248	3	407607	13	NULL	NULL	0	NULL	slow rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Subcutaneous infusions of gammaglobulin are usually given at a slow rate .
	manualset3
138249	1	407608	13	NULL	NULL	0	NULL	Subjective assessment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjective assessment of tiredness and dryness of mouth were measured by using visual analog scales ( VAS ) .
	manualset3
138250	2	407608	13	NULL	NULL	0	NULL	tiredness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjective assessment of tiredness and dryness of mouth were measured by using visual analog scales ( VAS ) .
	manualset3
138251	3	407608	13	NULL	NULL	0	NULL	dryness of mouth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjective assessment of tiredness and dryness of mouth were measured by using visual analog scales ( VAS ) .
	manualset3
138252	4	407608	13	NULL	NULL	0	NULL	visual analog scales ( VAS )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjective assessment of tiredness and dryness of mouth were measured by using visual analog scales ( VAS ) .
	manualset3
138253	1	407609	13	NULL	NULL	0	NULL	Subjective health-related quality of life ( HRQoL ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjective health-related quality of life ( HRQoL ) was investigated in 100 patients with disturbed sleep ( 39 women aged 52 + / - 13 years and 61 men aged 53 + / - 10 years ) referred to the sleep laboratory and compared with HRQoL in 100 normal healthy adults .
	manualset3
138254	2	407609	13	NULL	NULL	0	NULL	100 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjective health-related quality of life ( HRQoL ) was investigated in 100 patients with disturbed sleep ( 39 women aged 52 + / - 13 years and 61 men aged 53 + / - 10 years ) referred to the sleep laboratory and compared with HRQoL in 100 normal healthy adults .
	manualset3
138255	3	407609	13	NULL	NULL	0	NULL	39 women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjective health-related quality of life ( HRQoL ) was investigated in 100 patients with disturbed sleep ( 39 women aged 52 + / - 13 years and 61 men aged 53 + / - 10 years ) referred to the sleep laboratory and compared with HRQoL in 100 normal healthy adults .
	manualset3
138256	4	407609	13	NULL	NULL	0	NULL	aged 52 + / - 13 years	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjective health-related quality of life ( HRQoL ) was investigated in 100 patients with disturbed sleep ( 39 women aged 52 + / - 13 years and 61 men aged 53 + / - 10 years ) referred to the sleep laboratory and compared with HRQoL in 100 normal healthy adults .
	manualset3
138257	5	407609	13	NULL	NULL	0	NULL	61 men 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjective health-related quality of life ( HRQoL ) was investigated in 100 patients with disturbed sleep ( 39 women aged 52 + / - 13 years and 61 men aged 53 + / - 10 years ) referred to the sleep laboratory and compared with HRQoL in 100 normal healthy adults .
	manualset3
138258	6	407609	13	NULL	NULL	0	NULL	aged 53 + / - 10 years	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjective health-related quality of life ( HRQoL ) was investigated in 100 patients with disturbed sleep ( 39 women aged 52 + / - 13 years and 61 men aged 53 + / - 10 years ) referred to the sleep laboratory and compared with HRQoL in 100 normal healthy adults .
	manualset3
138259	7	407609	13	NULL	NULL	0	NULL	sleep laboratory	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjective health-related quality of life ( HRQoL ) was investigated in 100 patients with disturbed sleep ( 39 women aged 52 + / - 13 years and 61 men aged 53 + / - 10 years ) referred to the sleep laboratory and compared with HRQoL in 100 normal healthy adults .
	manualset3
138260	8	407609	13	NULL	NULL	0	NULL	HRQoL	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjective health-related quality of life ( HRQoL ) was investigated in 100 patients with disturbed sleep ( 39 women aged 52 + / - 13 years and 61 men aged 53 + / - 10 years ) referred to the sleep laboratory and compared with HRQoL in 100 normal healthy adults .
	manualset3
138261	9	407609	13	NULL	NULL	0	NULL	100 normal healthy adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjective health-related quality of life ( HRQoL ) was investigated in 100 patients with disturbed sleep ( 39 women aged 52 + / - 13 years and 61 men aged 53 + / - 10 years ) referred to the sleep laboratory and compared with HRQoL in 100 normal healthy adults .
	manualset3
138262	1	407610	13	NULL	NULL	0	NULL	Subjectivity	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjectivity and culpability in the constitution of nurse-patient relationships .
	manualset3
138263	2	407610	13	NULL	NULL	0	NULL	culpability 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjectivity and culpability in the constitution of nurse-patient relationships .
	manualset3
138264	3	407610	13	NULL	NULL	0	NULL	constitution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjectivity and culpability in the constitution of nurse-patient relationships .
	manualset3
138265	4	407610	13	NULL	NULL	0	NULL	nurse-patient relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjectivity and culpability in the constitution of nurse-patient relationships .
	manualset3
138266	1	407611	13	NULL	NULL	0	NULL	Subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects did not make saccades to the position they tapped but kept pursuing the disk .
	manualset3
138267	2	407611	13	NULL	NULL	0	NULL	saccades	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects did not make saccades to the position they tapped but kept pursuing the disk .
	manualset3
138268	3	407611	13	NULL	NULL	0	NULL	position 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects did not make saccades to the position they tapped but kept pursuing the disk .
	manualset3
138269	4	407611	13	NULL	NULL	0	NULL	disk 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects did not make saccades to the position they tapped but kept pursuing the disk .
	manualset3
138270	1	407612	13	NULL	NULL	0	NULL	Subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects rated their levels of leisure and occupational activities .
	manualset3
138271	2	407612	13	NULL	NULL	0	NULL	levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects rated their levels of leisure and occupational activities .
	manualset3
138272	3	407612	13	NULL	NULL	0	NULL	leisure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects rated their levels of leisure and occupational activities .
	manualset3
138273	4	407612	13	NULL	NULL	0	NULL	occupational activities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects rated their levels of leisure and occupational activities .
	manualset3
138274	1	407613	13	NULL	NULL	0	NULL	Subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were administered tests of primary memory ( digit span ) and tests of secondary memory with immediate and delayed recall components ( paragraph , paired associate , list recall ; facial recognition ) .
	manualset3
138275	2	407613	13	NULL	NULL	0	NULL	tests of primary memory	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were administered tests of primary memory ( digit span ) and tests of secondary memory with immediate and delayed recall components ( paragraph , paired associate , list recall ; facial recognition ) .
	manualset3
138276	3	407613	13	NULL	NULL	0	NULL	digit span	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were administered tests of primary memory ( digit span ) and tests of secondary memory with immediate and delayed recall components ( paragraph , paired associate , list recall ; facial recognition ) .
	manualset3
138277	4	407613	13	NULL	NULL	0	NULL	tests of secondary memory	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were administered tests of primary memory ( digit span ) and tests of secondary memory with immediate and delayed recall components ( paragraph , paired associate , list recall ; facial recognition ) .
	manualset3
138278	5	407613	13	NULL	NULL	0	NULL	components	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were administered tests of primary memory ( digit span ) and tests of secondary memory with immediate and delayed recall components ( paragraph , paired associate , list recall ; facial recognition ) .
	manualset3
138279	6	407613	13	NULL	NULL	0	NULL	paragraph	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were administered tests of primary memory ( digit span ) and tests of secondary memory with immediate and delayed recall components ( paragraph , paired associate , list recall ; facial recognition ) .
	manualset3
138280	7	407613	13	NULL	NULL	0	NULL	paired associate	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were administered tests of primary memory ( digit span ) and tests of secondary memory with immediate and delayed recall components ( paragraph , paired associate , list recall ; facial recognition ) .
	manualset3
138281	8	407613	13	NULL	NULL	0	NULL	list recall 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were administered tests of primary memory ( digit span ) and tests of secondary memory with immediate and delayed recall components ( paragraph , paired associate , list recall ; facial recognition ) .
	manualset3
138282	9	407613	13	NULL	NULL	0	NULL	facial recognition 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were administered tests of primary memory ( digit span ) and tests of secondary memory with immediate and delayed recall components ( paragraph , paired associate , list recall ; facial recognition ) .
	manualset3
138283	1	407614	13	NULL	NULL	0	NULL	Subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were assigned to one of two groups ( n = 9 ) for weight-training only or for combined pendulum and weight-training .
	manualset3
138284	2	407614	13	NULL	NULL	0	NULL	one of two groups	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were assigned to one of two groups ( n = 9 ) for weight-training only or for combined pendulum and weight-training .
	manualset3
138285	3	407614	13	NULL	NULL	0	NULL	n = 9 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were assigned to one of two groups ( n = 9 ) for weight-training only or for combined pendulum and weight-training .
	manualset3
138286	4	407614	13	NULL	NULL	0	NULL	pendulum	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were assigned to one of two groups ( n = 9 ) for weight-training only or for combined pendulum and weight-training .
	manualset3
138438	5	407614	13	NULL	NULL	0	NULL	weight-training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were assigned to one of two groups ( n = 9 ) for weight-training only or for combined pendulum and weight-training .
	manualset3
138439	6	407614	13	NULL	NULL	0	NULL	weight-training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were assigned to one of two groups ( n = 9 ) for weight-training only or for combined pendulum and weight-training .
	manualset3
138287	1	407615	13	NULL	NULL	0	NULL	Subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were divided into 3 groups : LD , HD , and placebo ( P ) .
	manualset3
138288	2	407615	13	NULL	NULL	NULL	NULL	3 groups 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Subjects were divided into 3 groups : LD , HD , and placebo ( P ) .
	manualset3
138289	3	407615	13	NULL	NULL	0	NULL	LD	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were divided into 3 groups : LD , HD , and placebo ( P ) .
	manualset3
138290	4	407615	13	NULL	NULL	0	NULL	HD	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were divided into 3 groups : LD , HD , and placebo ( P ) .
	manualset3
138291	5	407615	13	NULL	NULL	0	NULL	placebo ( P ) 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were divided into 3 groups : LD , HD , and placebo ( P ) .
	manualset3
138292	1	407616	13	NULL	NULL	0	NULL	Subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were included when their CD4 + cell count was less than 100/mm3 .
	manualset3
138293	2	407616	13	NULL	NULL	0	NULL	CD4 + cell count	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were included when their CD4 + cell count was less than 100/mm3 .
	manualset3
138294	3	407616	13	NULL	NULL	0	NULL	less than 100/mm3	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were included when their CD4 + cell count was less than 100/mm3 .
	manualset3
138295	1	407617	13	NULL	NULL	0	NULL	Subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were instructed to respond according to the meaning of the stimulus in the ( WORD task ) , to the case in which the stimulus was written ( CASE task ) , or to both the case and meaning of the stimulus ( CASE/WORD ) task .
	manualset3
138296	2	407617	13	NULL	NULL	0	NULL	meaning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were instructed to respond according to the meaning of the stimulus in the ( WORD task ) , to the case in which the stimulus was written ( CASE task ) , or to both the case and meaning of the stimulus ( CASE/WORD ) task .
	manualset3
138297	3	407617	13	NULL	NULL	0	NULL	stimulus 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were instructed to respond according to the meaning of the stimulus in the ( WORD task ) , to the case in which the stimulus was written ( CASE task ) , or to both the case and meaning of the stimulus ( CASE/WORD ) task .
	manualset3
138298	4	407617	13	NULL	NULL	0	NULL	WORD task	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were instructed to respond according to the meaning of the stimulus in the ( WORD task ) , to the case in which the stimulus was written ( CASE task ) , or to both the case and meaning of the stimulus ( CASE/WORD ) task .
	manualset3
138299	5	407617	13	NULL	NULL	0	NULL	case 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were instructed to respond according to the meaning of the stimulus in the ( WORD task ) , to the case in which the stimulus was written ( CASE task ) , or to both the case and meaning of the stimulus ( CASE/WORD ) task .
	manualset3
138300	6	407617	13	NULL	NULL	0	NULL	stimulus	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were instructed to respond according to the meaning of the stimulus in the ( WORD task ) , to the case in which the stimulus was written ( CASE task ) , or to both the case and meaning of the stimulus ( CASE/WORD ) task .
	manualset3
138301	7	407617	13	NULL	NULL	0	NULL	CASE task	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were instructed to respond according to the meaning of the stimulus in the ( WORD task ) , to the case in which the stimulus was written ( CASE task ) , or to both the case and meaning of the stimulus ( CASE/WORD ) task .
	manualset3
138302	8	407617	13	NULL	NULL	0	NULL	case	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were instructed to respond according to the meaning of the stimulus in the ( WORD task ) , to the case in which the stimulus was written ( CASE task ) , or to both the case and meaning of the stimulus ( CASE/WORD ) task .
	manualset3
138303	9	407617	13	NULL	NULL	0	NULL	meaning 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were instructed to respond according to the meaning of the stimulus in the ( WORD task ) , to the case in which the stimulus was written ( CASE task ) , or to both the case and meaning of the stimulus ( CASE/WORD ) task .
	manualset3
138304	10	407617	13	NULL	NULL	0	NULL	stimulus	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were instructed to respond according to the meaning of the stimulus in the ( WORD task ) , to the case in which the stimulus was written ( CASE task ) , or to both the case and meaning of the stimulus ( CASE/WORD ) task .
	manualset3
138305	11	407617	13	NULL	NULL	0	NULL	( CASE/WORD ) task 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were instructed to respond according to the meaning of the stimulus in the ( WORD task ) , to the case in which the stimulus was written ( CASE task ) , or to both the case and meaning of the stimulus ( CASE/WORD ) task .
	manualset3
138306	1	407618	13	NULL	NULL	0	NULL	Subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were tested in three sessions , separated by 1 week , for short-term changes in blood variables , indirect calorimetry , subjective performance and different objective performance tasks using a repeated-measures counterbalanced cross-over design .
	manualset3
138307	2	407618	13	NULL	NULL	0	NULL	three sessions	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were tested in three sessions , separated by 1 week , for short-term changes in blood variables , indirect calorimetry , subjective performance and different objective performance tasks using a repeated-measures counterbalanced cross-over design .
	manualset3
138308	3	407618	13	NULL	NULL	0	NULL	1 week	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were tested in three sessions , separated by 1 week , for short-term changes in blood variables , indirect calorimetry , subjective performance and different objective performance tasks using a repeated-measures counterbalanced cross-over design .
	manualset3
138309	4	407618	13	NULL	NULL	0	NULL	short-term changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were tested in three sessions , separated by 1 week , for short-term changes in blood variables , indirect calorimetry , subjective performance and different objective performance tasks using a repeated-measures counterbalanced cross-over design .
	manualset3
138310	5	407618	13	NULL	NULL	0	NULL	blood variables	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were tested in three sessions , separated by 1 week , for short-term changes in blood variables , indirect calorimetry , subjective performance and different objective performance tasks using a repeated-measures counterbalanced cross-over design .
	manualset3
138311	6	407618	13	NULL	NULL	0	NULL	indirect calorimetry	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were tested in three sessions , separated by 1 week , for short-term changes in blood variables , indirect calorimetry , subjective performance and different objective performance tasks using a repeated-measures counterbalanced cross-over design .
	manualset3
138312	7	407618	13	NULL	NULL	0	NULL	subjective performance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were tested in three sessions , separated by 1 week , for short-term changes in blood variables , indirect calorimetry , subjective performance and different objective performance tasks using a repeated-measures counterbalanced cross-over design .
	manualset3
138313	8	407618	13	NULL	NULL	0	NULL	objective performance tasks	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were tested in three sessions , separated by 1 week , for short-term changes in blood variables , indirect calorimetry , subjective performance and different objective performance tasks using a repeated-measures counterbalanced cross-over design .
	manualset3
138314	9	407618	13	NULL	NULL	NULL	NULL	repeated-measures counterbalanced cross-over design	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Subjects were tested in three sessions , separated by 1 week , for short-term changes in blood variables , indirect calorimetry , subjective performance and different objective performance tasks using a repeated-measures counterbalanced cross-over design .
	manualset3
138315	1	407619	13	NULL	NULL	0	NULL	Subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects who had never walked or stopped walking 4-64 years prior to this study still experience walking in their dreams , suggesting that a cerebral walking program , either genetic or more probably developed via mirror neurons ( activated when observing others performing an action ) is reactivated during sleep .
	manualset3
138316	2	407619	13	NULL	NULL	0	NULL	4-64 years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects who had never walked or stopped walking 4-64 years prior to this study still experience walking in their dreams , suggesting that a cerebral walking program , either genetic or more probably developed via mirror neurons ( activated when observing others performing an action ) is reactivated during sleep .
	manualset3
138317	3	407619	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects who had never walked or stopped walking 4-64 years prior to this study still experience walking in their dreams , suggesting that a cerebral walking program , either genetic or more probably developed via mirror neurons ( activated when observing others performing an action ) is reactivated during sleep .
	manualset3
138318	4	407619	13	NULL	NULL	0	NULL	experience 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects who had never walked or stopped walking 4-64 years prior to this study still experience walking in their dreams , suggesting that a cerebral walking program , either genetic or more probably developed via mirror neurons ( activated when observing others performing an action ) is reactivated during sleep .
	manualset3
138319	5	407619	13	NULL	NULL	0	NULL	dreams	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects who had never walked or stopped walking 4-64 years prior to this study still experience walking in their dreams , suggesting that a cerebral walking program , either genetic or more probably developed via mirror neurons ( activated when observing others performing an action ) is reactivated during sleep .
	manualset3
138320	6	407619	13	NULL	NULL	0	NULL	cerebral walking program	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects who had never walked or stopped walking 4-64 years prior to this study still experience walking in their dreams , suggesting that a cerebral walking program , either genetic or more probably developed via mirror neurons ( activated when observing others performing an action ) is reactivated during sleep .
	manualset3
138321	7	407619	13	NULL	NULL	0	NULL	mirror neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects who had never walked or stopped walking 4-64 years prior to this study still experience walking in their dreams , suggesting that a cerebral walking program , either genetic or more probably developed via mirror neurons ( activated when observing others performing an action ) is reactivated during sleep .
	manualset3
138322	8	407619	13	NULL	NULL	0	NULL	others	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects who had never walked or stopped walking 4-64 years prior to this study still experience walking in their dreams , suggesting that a cerebral walking program , either genetic or more probably developed via mirror neurons ( activated when observing others performing an action ) is reactivated during sleep .
	manualset3
138323	9	407619	13	NULL	NULL	0	NULL	action	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects who had never walked or stopped walking 4-64 years prior to this study still experience walking in their dreams , suggesting that a cerebral walking program , either genetic or more probably developed via mirror neurons ( activated when observing others performing an action ) is reactivated during sleep .
	manualset3
138324	10	407619	13	NULL	NULL	0	NULL	sleep	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects who had never walked or stopped walking 4-64 years prior to this study still experience walking in their dreams , suggesting that a cerebral walking program , either genetic or more probably developed via mirror neurons ( activated when observing others performing an action ) is reactivated during sleep .
	manualset3
138440	11	407619	13	NULL	NULL	0	NULL	walking	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects who had never walked or stopped walking 4-64 years prior to this study still experience walking in their dreams , suggesting that a cerebral walking program , either genetic or more probably developed via mirror neurons ( activated when observing others performing an action ) is reactivated during sleep .
	manualset3
138325	1	407620	13	NULL	NULL	0	NULL	Subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects with a history of CV or cerebrovascular disease have an even greater CV risk if microalbuminuria is present than if it is not ; however , in all cases , therapeutic intervention must be aggressive regardless of whether microalbuminuria is present or not .
	manualset3
138326	2	407620	13	NULL	NULL	0	NULL	history of CV 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects with a history of CV or cerebrovascular disease have an even greater CV risk if microalbuminuria is present than if it is not ; however , in all cases , therapeutic intervention must be aggressive regardless of whether microalbuminuria is present or not .
	manualset3
138327	3	407620	13	NULL	NULL	0	NULL	cerebrovascular disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects with a history of CV or cerebrovascular disease have an even greater CV risk if microalbuminuria is present than if it is not ; however , in all cases , therapeutic intervention must be aggressive regardless of whether microalbuminuria is present or not .
	manualset3
138328	4	407620	13	NULL	NULL	0	NULL	CV risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects with a history of CV or cerebrovascular disease have an even greater CV risk if microalbuminuria is present than if it is not ; however , in all cases , therapeutic intervention must be aggressive regardless of whether microalbuminuria is present or not .
	manualset3
138329	5	407620	13	NULL	NULL	0	NULL	microalbuminuria 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects with a history of CV or cerebrovascular disease have an even greater CV risk if microalbuminuria is present than if it is not ; however , in all cases , therapeutic intervention must be aggressive regardless of whether microalbuminuria is present or not .
	manualset3
138330	6	407620	13	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects with a history of CV or cerebrovascular disease have an even greater CV risk if microalbuminuria is present than if it is not ; however , in all cases , therapeutic intervention must be aggressive regardless of whether microalbuminuria is present or not .
	manualset3
138331	7	407620	13	NULL	NULL	0	NULL	therapeutic intervention 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects with a history of CV or cerebrovascular disease have an even greater CV risk if microalbuminuria is present than if it is not ; however , in all cases , therapeutic intervention must be aggressive regardless of whether microalbuminuria is present or not .
	manualset3
138332	8	407620	13	NULL	NULL	0	NULL	microalbuminuria	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects with a history of CV or cerebrovascular disease have an even greater CV risk if microalbuminuria is present than if it is not ; however , in all cases , therapeutic intervention must be aggressive regardless of whether microalbuminuria is present or not .
	manualset3
138333	1	407621	13	NULL	NULL	0	NULL	Subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects wrote down their spontaneous reactions to six film personalities , divided over three clips , including what they thought to be characteristic traits of these persons .
	manualset3
138334	2	407621	13	NULL	NULL	0	NULL	spontaneous reactions	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects wrote down their spontaneous reactions to six film personalities , divided over three clips , including what they thought to be characteristic traits of these persons .
	manualset3
138335	3	407621	13	NULL	NULL	0	NULL	six film personalities	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects wrote down their spontaneous reactions to six film personalities , divided over three clips , including what they thought to be characteristic traits of these persons .
	manualset3
138336	4	407621	13	NULL	NULL	0	NULL	three clips 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects wrote down their spontaneous reactions to six film personalities , divided over three clips , including what they thought to be characteristic traits of these persons .
	manualset3
138337	5	407621	13	NULL	NULL	0	NULL	characteristic traits 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects wrote down their spontaneous reactions to six film personalities , divided over three clips , including what they thought to be characteristic traits of these persons .
	manualset3
138338	6	407621	13	NULL	NULL	0	NULL	persons	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects wrote down their spontaneous reactions to six film personalities , divided over three clips , including what they thought to be characteristic traits of these persons .
	manualset3
138339	1	407622	13	NULL	NULL	0	NULL	Suboptimal pain relief	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Suboptimal pain relief administered during CMR should prompt positive actions to ensure that the patient is not subjected to undue pain just for the sake of an acceptable fracture reduction .
	manualset3
138340	2	407622	13	NULL	NULL	0	NULL	CMR	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Suboptimal pain relief administered during CMR should prompt positive actions to ensure that the patient is not subjected to undue pain just for the sake of an acceptable fracture reduction .
	manualset3
138341	3	407622	13	NULL	NULL	0	NULL	positive actions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Suboptimal pain relief administered during CMR should prompt positive actions to ensure that the patient is not subjected to undue pain just for the sake of an acceptable fracture reduction .
	manualset3
138342	4	407622	13	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Suboptimal pain relief administered during CMR should prompt positive actions to ensure that the patient is not subjected to undue pain just for the sake of an acceptable fracture reduction .
	manualset3
138343	5	407622	13	NULL	NULL	0	NULL	undue pain 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Suboptimal pain relief administered during CMR should prompt positive actions to ensure that the patient is not subjected to undue pain just for the sake of an acceptable fracture reduction .
	manualset3
138344	6	407622	13	NULL	NULL	0	NULL	fracture reduction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Suboptimal pain relief administered during CMR should prompt positive actions to ensure that the patient is not subjected to undue pain just for the sake of an acceptable fracture reduction .
	manualset3
138345	1	407623	13	NULL	NULL	0	NULL	 3	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3 ) TNF alpha concentrations in the incubation medium were positively correlated with lipid peroxide concentrations , r = 0.608 .
	manualset3
138346	2	407623	13	NULL	NULL	0	NULL	TNF alpha concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3 ) TNF alpha concentrations in the incubation medium were positively correlated with lipid peroxide concentrations , r = 0.608 .
	manualset3
138347	3	407623	13	NULL	NULL	0	NULL	incubation medium 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3 ) TNF alpha concentrations in the incubation medium were positively correlated with lipid peroxide concentrations , r = 0.608 .
	manualset3
138348	4	407623	13	NULL	NULL	0	NULL	lipid peroxide concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3 ) TNF alpha concentrations in the incubation medium were positively correlated with lipid peroxide concentrations , r = 0.608 .
	manualset3
138349	5	407623	13	NULL	NULL	0	NULL	r = 0.608	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3 ) TNF alpha concentrations in the incubation medium were positively correlated with lipid peroxide concentrations , r = 0.608 .
	manualset3
138350	1	407624	13	NULL	NULL	0	NULL	Changes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Changes in body composition caused by intense physical training ) .
	manualset3
138351	2	407624	13	NULL	NULL	0	NULL	body composition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Changes in body composition caused by intense physical training ) .
	manualset3
138352	3	407624	13	NULL	NULL	0	NULL	physical training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Changes in body composition caused by intense physical training ) .
	manualset3
138353	1	407625	13	NULL	NULL	0	NULL	 mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A possible mechanism for collagen biosynthesis inhibition .
	manualset3
138354	2	407625	13	NULL	NULL	0	NULL	collagen biosynthesis inhibition 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A possible mechanism for collagen biosynthesis inhibition .
	manualset3
138355	1	407626	13	NULL	NULL	0	NULL	Suboptimal utilization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Suboptimal utilization of secondary drug prevention in acute coronary syndrome : measurement issues and managed care opportunities .
	manualset3
138356	2	407626	13	NULL	NULL	0	NULL	secondary drug prevention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Suboptimal utilization of secondary drug prevention in acute coronary syndrome : measurement issues and managed care opportunities .
	manualset3
138357	3	407626	13	NULL	NULL	0	NULL	acute coronary syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Suboptimal utilization of secondary drug prevention in acute coronary syndrome : measurement issues and managed care opportunities .
	manualset3
138358	4	407626	13	NULL	NULL	0	NULL	measurement issues 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Suboptimal utilization of secondary drug prevention in acute coronary syndrome : measurement issues and managed care opportunities .
	manualset3
138359	5	407626	13	NULL	NULL	0	NULL	care opportunities	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Suboptimal utilization of secondary drug prevention in acute coronary syndrome : measurement issues and managed care opportunities .
	manualset3
138360	1	407627	13	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent binding of ATP to the same GroEL ring causes rapid , forced unfolding of the substrate protein .
	manualset3
138361	2	407627	13	NULL	NULL	0	NULL	ATP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent binding of ATP to the same GroEL ring causes rapid , forced unfolding of the substrate protein .
	manualset3
138362	3	407627	13	NULL	NULL	0	NULL	GroEL ring	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent binding of ATP to the same GroEL ring causes rapid , forced unfolding of the substrate protein .
	manualset3
138363	4	407627	13	NULL	NULL	0	NULL	causes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent binding of ATP to the same GroEL ring causes rapid , forced unfolding of the substrate protein .
	manualset3
138364	5	407627	13	NULL	NULL	0	NULL	substrate protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent binding of ATP to the same GroEL ring causes rapid , forced unfolding of the substrate protein .
	manualset3
138441	6	407627	13	NULL	NULL	0	NULL	unfolding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent binding of ATP to the same GroEL ring causes rapid , forced unfolding of the substrate protein .
	manualset3
138365	1	407628	13	NULL	NULL	0	NULL	coronary angiography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent coronary angiography revealed the presence of 2 CAF , one extending from the left anterior descending artery to the pulmonary artery ( PA ) and the other extending from the proximal right coronary artery to the PA. .
	manualset3
138366	2	407628	13	NULL	NULL	0	NULL	presence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent coronary angiography revealed the presence of 2 CAF , one extending from the left anterior descending artery to the pulmonary artery ( PA ) and the other extending from the proximal right coronary artery to the PA. .
	manualset3
138367	3	407628	13	NULL	NULL	0	NULL	2 CAF 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent coronary angiography revealed the presence of 2 CAF , one extending from the left anterior descending artery to the pulmonary artery ( PA ) and the other extending from the proximal right coronary artery to the PA. .
	manualset3
138368	4	407628	13	NULL	NULL	0	NULL	left anterior descending artery 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent coronary angiography revealed the presence of 2 CAF , one extending from the left anterior descending artery to the pulmonary artery ( PA ) and the other extending from the proximal right coronary artery to the PA. .
	manualset3
138369	5	407628	13	NULL	NULL	0	NULL	pulmonary artery ( PA )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent coronary angiography revealed the presence of 2 CAF , one extending from the left anterior descending artery to the pulmonary artery ( PA ) and the other extending from the proximal right coronary artery to the PA. .
	manualset3
138370	6	407628	13	NULL	NULL	0	NULL	proximal right coronary artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent coronary angiography revealed the presence of 2 CAF , one extending from the left anterior descending artery to the pulmonary artery ( PA ) and the other extending from the proximal right coronary artery to the PA. .
	manualset3
138371	7	407628	13	NULL	NULL	0	NULL	PA	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent coronary angiography revealed the presence of 2 CAF , one extending from the left anterior descending artery to the pulmonary artery ( PA ) and the other extending from the proximal right coronary artery to the PA. .
	manualset3
138442	8	407628	13	NULL	NULL	0	NULL	extending	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent coronary angiography revealed the presence of 2 CAF , one extending from the left anterior descending artery to the pulmonary artery ( PA ) and the other extending from the proximal right coronary artery to the PA. .
	manualset3
138443	9	407628	13	NULL	NULL	0	NULL	extending	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent coronary angiography revealed the presence of 2 CAF , one extending from the left anterior descending artery to the pulmonary artery ( PA ) and the other extending from the proximal right coronary artery to the PA. .
	manualset3
138372	1	407629	13	NULL	NULL	0	NULL	Subsequent laparoscopic biopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent laparoscopic biopsy showed granulomatous inflammation , and tuberculosis polymerase chain reaction showed a positive result .
	manualset3
138373	2	407629	13	NULL	NULL	0	NULL	granulomatous inflammation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent laparoscopic biopsy showed granulomatous inflammation , and tuberculosis polymerase chain reaction showed a positive result .
	manualset3
138374	3	407629	13	NULL	NULL	0	NULL	tuberculosis polymerase chain reaction	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent laparoscopic biopsy showed granulomatous inflammation , and tuberculosis polymerase chain reaction showed a positive result .
	manualset3
138375	4	407629	13	NULL	NULL	0	NULL	positive result	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent laparoscopic biopsy showed granulomatous inflammation , and tuberculosis polymerase chain reaction showed a positive result .
	manualset3
138376	1	407630	13	NULL	NULL	0	NULL	Subsequent palladium-catalyzed Sonogashira reactions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent palladium-catalyzed Sonogashira , Suzuki , and Heck reactions of the resulting 3-iodoindoles proceed smoothly in good yields .
	manualset3
138377	2	407630	13	NULL	NULL	0	NULL	Subsequent palladium-catalyzed Suzuki reactions  	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent palladium-catalyzed Sonogashira , Suzuki , and Heck reactions of the resulting 3-iodoindoles proceed smoothly in good yields .
	manualset3
138378	3	407630	13	NULL	NULL	0	NULL	Subsequent palladium-catalyzed Heck reactions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent palladium-catalyzed Sonogashira , Suzuki , and Heck reactions of the resulting 3-iodoindoles proceed smoothly in good yields .
	manualset3
138379	4	407630	13	NULL	NULL	0	NULL	3-iodoindoles	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent palladium-catalyzed Sonogashira , Suzuki , and Heck reactions of the resulting 3-iodoindoles proceed smoothly in good yields .
	manualset3
138380	5	407630	13	NULL	NULL	0	NULL	good yields 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent palladium-catalyzed Sonogashira , Suzuki , and Heck reactions of the resulting 3-iodoindoles proceed smoothly in good yields .
	manualset3
138381	1	407631	13	NULL	NULL	0	NULL	passage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent passage in Vero cells resulted in a passage-8 virus which had increased neurovirulence with an LD ( 50 ) of 3.2 pfu/ml .
	manualset3
138382	2	407631	13	NULL	NULL	0	NULL	Vero cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent passage in Vero cells resulted in a passage-8 virus which had increased neurovirulence with an LD ( 50 ) of 3.2 pfu/ml .
	manualset3
138383	3	407631	13	NULL	NULL	0	NULL	passage-8 virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent passage in Vero cells resulted in a passage-8 virus which had increased neurovirulence with an LD ( 50 ) of 3.2 pfu/ml .
	manualset3
138384	4	407631	13	NULL	NULL	0	NULL	neurovirulence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent passage in Vero cells resulted in a passage-8 virus which had increased neurovirulence with an LD ( 50 ) of 3.2 pfu/ml .
	manualset3
138385	5	407631	13	NULL	NULL	0	NULL	LD ( 50 ) of 3.2 pfu/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent passage in Vero cells resulted in a passage-8 virus which had increased neurovirulence with an LD ( 50 ) of 3.2 pfu/ml .
	manualset3
138386	1	407632	13	NULL	NULL	0	NULL	Subsequent patch testing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent patch testing revealed positive reactions to both the POP bandage used and to benzalkonium chloride , a component of the POP formulation .
	manualset3
138387	2	407632	13	NULL	NULL	0	NULL	positive reactions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent patch testing revealed positive reactions to both the POP bandage used and to benzalkonium chloride , a component of the POP formulation .
	manualset3
138388	3	407632	13	NULL	NULL	0	NULL	POP bandage	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent patch testing revealed positive reactions to both the POP bandage used and to benzalkonium chloride , a component of the POP formulation .
	manualset3
138389	4	407632	13	NULL	NULL	0	NULL	benzalkonium chloride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent patch testing revealed positive reactions to both the POP bandage used and to benzalkonium chloride , a component of the POP formulation .
	manualset3
138390	5	407632	13	NULL	NULL	0	NULL	component	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent patch testing revealed positive reactions to both the POP bandage used and to benzalkonium chloride , a component of the POP formulation .
	manualset3
138391	6	407632	13	NULL	NULL	0	NULL	POP formulation 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent patch testing revealed positive reactions to both the POP bandage used and to benzalkonium chloride , a component of the POP formulation .
	manualset3
138392	1	407633	13	NULL	NULL	0	NULL	Subsequent sequencing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent sequencing revealed a new VEGF isoform formed by differential splicing from the end of exon 7 into the 3 ' untranslated region of the mRNA .
	manualset3
138393	2	407633	13	NULL	NULL	0	NULL	VEGF isoform	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent sequencing revealed a new VEGF isoform formed by differential splicing from the end of exon 7 into the 3 ' untranslated region of the mRNA .
	manualset3
138394	3	407633	13	NULL	NULL	0	NULL	end of exon 7 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent sequencing revealed a new VEGF isoform formed by differential splicing from the end of exon 7 into the 3 ' untranslated region of the mRNA .
	manualset3
138395	4	407633	13	NULL	NULL	0	NULL	3 ' untranslated region of the mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent sequencing revealed a new VEGF isoform formed by differential splicing from the end of exon 7 into the 3 ' untranslated region of the mRNA .
	manualset3
138396	1	407634	13	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent to the application of SR 141716A , the Ca ( 2 + ) current inhibition by NE and SOM was abolished .
	manualset3
138397	2	407634	13	NULL	NULL	NULL	NULL	 SR 141716A	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Subsequent to the application of SR 141716A , the Ca ( 2 + ) current inhibition by NE and SOM was abolished .
	manualset3
138398	3	407634	13	NULL	NULL	0	NULL	Ca ( 2 + ) current inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent to the application of SR 141716A , the Ca ( 2 + ) current inhibition by NE and SOM was abolished .
	manualset3
138399	4	407634	13	NULL	NULL	0	NULL	NE	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent to the application of SR 141716A , the Ca ( 2 + ) current inhibition by NE and SOM was abolished .
	manualset3
138400	5	407634	13	NULL	NULL	0	NULL	SOM 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent to the application of SR 141716A , the Ca ( 2 + ) current inhibition by NE and SOM was abolished .
	manualset3
138401	1	407635	13	NULL	NULL	0	NULL	appointment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent to the appointment of an anemia research nurse a base-line audit revealed that only 61.3 % of the dialysis population had a hemoglobin ) 10 g/dl and also identified the reasons why the unit was failing to meet this pre-set target .
	manualset3
138402	2	407635	13	NULL	NULL	0	NULL	anemia research nurse 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent to the appointment of an anemia research nurse a base-line audit revealed that only 61.3 % of the dialysis population had a hemoglobin ) 10 g/dl and also identified the reasons why the unit was failing to meet this pre-set target .
	manualset3
138403	3	407635	13	NULL	NULL	0	NULL	base-line audit	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent to the appointment of an anemia research nurse a base-line audit revealed that only 61.3 % of the dialysis population had a hemoglobin ) 10 g/dl and also identified the reasons why the unit was failing to meet this pre-set target .
	manualset3
138404	4	407635	13	NULL	NULL	0	NULL	61.3 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent to the appointment of an anemia research nurse a base-line audit revealed that only 61.3 % of the dialysis population had a hemoglobin ) 10 g/dl and also identified the reasons why the unit was failing to meet this pre-set target .
	manualset3
138405	5	407635	13	NULL	NULL	0	NULL	dialysis population 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent to the appointment of an anemia research nurse a base-line audit revealed that only 61.3 % of the dialysis population had a hemoglobin ) 10 g/dl and also identified the reasons why the unit was failing to meet this pre-set target .
	manualset3
138406	6	407635	13	NULL	NULL	0	NULL	hemoglobin ) 10 g/dl	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent to the appointment of an anemia research nurse a base-line audit revealed that only 61.3 % of the dialysis population had a hemoglobin ) 10 g/dl and also identified the reasons why the unit was failing to meet this pre-set target .
	manualset3
138407	7	407635	13	NULL	NULL	0	NULL	reasons	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent to the appointment of an anemia research nurse a base-line audit revealed that only 61.3 % of the dialysis population had a hemoglobin ) 10 g/dl and also identified the reasons why the unit was failing to meet this pre-set target .
	manualset3
138408	8	407635	13	NULL	NULL	0	NULL	unit 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent to the appointment of an anemia research nurse a base-line audit revealed that only 61.3 % of the dialysis population had a hemoglobin ) 10 g/dl and also identified the reasons why the unit was failing to meet this pre-set target .
	manualset3
138409	9	407635	13	NULL	NULL	0	NULL	pre-set target	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent to the appointment of an anemia research nurse a base-line audit revealed that only 61.3 % of the dialysis population had a hemoglobin ) 10 g/dl and also identified the reasons why the unit was failing to meet this pre-set target .
	manualset3
138410	1	407636	13	NULL	NULL	0	NULL	generation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent to the generation of ustekinumab , it was discovered that IL-23 also contains the p40 subunit .
	manualset3
138411	2	407636	13	NULL	NULL	0	NULL	ustekinumab	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent to the generation of ustekinumab , it was discovered that IL-23 also contains the p40 subunit .
	manualset3
138412	3	407636	13	NULL	NULL	0	NULL	IL-23	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent to the generation of ustekinumab , it was discovered that IL-23 also contains the p40 subunit .
	manualset3
138413	4	407636	13	NULL	NULL	0	NULL	p40 subunit	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent to the generation of ustekinumab , it was discovered that IL-23 also contains the p40 subunit .
	manualset3
138414	1	407637	13	NULL	NULL	0	NULL	telomerase reverse transcriptase RNA-template ( guide RNA ) 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , annealing of the telomerase reverse transcriptase RNA-template ( guide RNA ) at short regions of homology is followed by extension of the nascent 3 ' - end of the broken chromosome to copy a short region of the telomerase guide RNA ; multiple cycles of this process yield the new telomere .
	manualset3
138415	2	407637	13	NULL	NULL	0	NULL	short regions	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , annealing of the telomerase reverse transcriptase RNA-template ( guide RNA ) at short regions of homology is followed by extension of the nascent 3 ' - end of the broken chromosome to copy a short region of the telomerase guide RNA ; multiple cycles of this process yield the new telomere .
	manualset3
138416	3	407637	13	NULL	NULL	0	NULL	homology 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , annealing of the telomerase reverse transcriptase RNA-template ( guide RNA ) at short regions of homology is followed by extension of the nascent 3 ' - end of the broken chromosome to copy a short region of the telomerase guide RNA ; multiple cycles of this process yield the new telomere .
	manualset3
138417	4	407637	13	NULL	NULL	0	NULL	extension of the nascent 3 ' - end	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , annealing of the telomerase reverse transcriptase RNA-template ( guide RNA ) at short regions of homology is followed by extension of the nascent 3 ' - end of the broken chromosome to copy a short region of the telomerase guide RNA ; multiple cycles of this process yield the new telomere .
	manualset3
138418	5	407637	13	NULL	NULL	0	NULL	chromosome	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , annealing of the telomerase reverse transcriptase RNA-template ( guide RNA ) at short regions of homology is followed by extension of the nascent 3 ' - end of the broken chromosome to copy a short region of the telomerase guide RNA ; multiple cycles of this process yield the new telomere .
	manualset3
138419	6	407637	13	NULL	NULL	0	NULL	short region 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , annealing of the telomerase reverse transcriptase RNA-template ( guide RNA ) at short regions of homology is followed by extension of the nascent 3 ' - end of the broken chromosome to copy a short region of the telomerase guide RNA ; multiple cycles of this process yield the new telomere .
	manualset3
138420	7	407637	13	NULL	NULL	0	NULL	telomerase guide RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , annealing of the telomerase reverse transcriptase RNA-template ( guide RNA ) at short regions of homology is followed by extension of the nascent 3 ' - end of the broken chromosome to copy a short region of the telomerase guide RNA ; multiple cycles of this process yield the new telomere .
	manualset3
138421	8	407637	13	NULL	NULL	0	NULL	multiple cycles	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , annealing of the telomerase reverse transcriptase RNA-template ( guide RNA ) at short regions of homology is followed by extension of the nascent 3 ' - end of the broken chromosome to copy a short region of the telomerase guide RNA ; multiple cycles of this process yield the new telomere .
	manualset3
138422	9	407637	13	NULL	NULL	0	NULL	process	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , annealing of the telomerase reverse transcriptase RNA-template ( guide RNA ) at short regions of homology is followed by extension of the nascent 3 ' - end of the broken chromosome to copy a short region of the telomerase guide RNA ; multiple cycles of this process yield the new telomere .
	manualset3
138423	10	407637	13	NULL	NULL	0	NULL	yield	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , annealing of the telomerase reverse transcriptase RNA-template ( guide RNA ) at short regions of homology is followed by extension of the nascent 3 ' - end of the broken chromosome to copy a short region of the telomerase guide RNA ; multiple cycles of this process yield the new telomere .
	manualset3
138424	11	407637	13	NULL	NULL	0	NULL	telomere	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , annealing of the telomerase reverse transcriptase RNA-template ( guide RNA ) at short regions of homology is followed by extension of the nascent 3 ' - end of the broken chromosome to copy a short region of the telomerase guide RNA ; multiple cycles of this process yield the new telomere .
	manualset3
151650	12	407637	13	NULL	NULL	0	NULL	annealing 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , annealing of the telomerase reverse transcriptase RNA-template ( guide RNA ) at short regions of homology is followed by extension of the nascent 3 ' - end of the broken chromosome to copy a short region of the telomerase guide RNA ; multiple cycles of this process yield the new telomere .
	manualset3
148676	1	407638	13	NULL	NULL	0	NULL	prostate cancer skeletal metastasis mouse model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , in a prostate cancer skeletal metastasis mouse model , PTHrP-knockdown PC-3 cells resulted in significantly fewer metastatic lesions compared to control PC-3 cells , suggesting that PTHrP mediated antianoikis events in the bloodstream .
	manualset3
148677	2	407638	13	NULL	NULL	0	NULL	PTHrP-knockdown PC-3 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , in a prostate cancer skeletal metastasis mouse model , PTHrP-knockdown PC-3 cells resulted in significantly fewer metastatic lesions compared to control PC-3 cells , suggesting that PTHrP mediated antianoikis events in the bloodstream .
	manualset3
148678	3	407638	13	NULL	NULL	0	NULL	metastatic lesions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , in a prostate cancer skeletal metastasis mouse model , PTHrP-knockdown PC-3 cells resulted in significantly fewer metastatic lesions compared to control PC-3 cells , suggesting that PTHrP mediated antianoikis events in the bloodstream .
	manualset3
148679	4	407638	13	NULL	NULL	0	NULL	control PC-3 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , in a prostate cancer skeletal metastasis mouse model , PTHrP-knockdown PC-3 cells resulted in significantly fewer metastatic lesions compared to control PC-3 cells , suggesting that PTHrP mediated antianoikis events in the bloodstream .
	manualset3
148680	5	407638	13	NULL	NULL	0	NULL	PTHrP	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , in a prostate cancer skeletal metastasis mouse model , PTHrP-knockdown PC-3 cells resulted in significantly fewer metastatic lesions compared to control PC-3 cells , suggesting that PTHrP mediated antianoikis events in the bloodstream .
	manualset3
148681	6	407638	13	NULL	NULL	0	NULL	antianoikis events	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , in a prostate cancer skeletal metastasis mouse model , PTHrP-knockdown PC-3 cells resulted in significantly fewer metastatic lesions compared to control PC-3 cells , suggesting that PTHrP mediated antianoikis events in the bloodstream .
	manualset3
148682	7	407638	13	NULL	NULL	0	NULL	bloodstream 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , in a prostate cancer skeletal metastasis mouse model , PTHrP-knockdown PC-3 cells resulted in significantly fewer metastatic lesions compared to control PC-3 cells , suggesting that PTHrP mediated antianoikis events in the bloodstream .
	manualset3
148683	1	407639	13	NULL	NULL	0	NULL	graphene microflakes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , individual graphene microflakes can be picked up and transferred to a target hole on a suspended SiN membrane with 1m precision via a site-specific transfer-printing method .
	manualset3
148684	2	407639	13	NULL	NULL	0	NULL	target hole	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , individual graphene microflakes can be picked up and transferred to a target hole on a suspended SiN membrane with 1m precision via a site-specific transfer-printing method .
	manualset3
148685	3	407639	13	NULL	NULL	0	NULL	SiN membrane	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , individual graphene microflakes can be picked up and transferred to a target hole on a suspended SiN membrane with 1m precision via a site-specific transfer-printing method .
	manualset3
148686	4	407639	13	NULL	NULL	0	NULL	1m precision 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , individual graphene microflakes can be picked up and transferred to a target hole on a suspended SiN membrane with 1m precision via a site-specific transfer-printing method .
	manualset3
148687	5	407639	13	NULL	NULL	0	NULL	site-specific transfer-printing method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , individual graphene microflakes can be picked up and transferred to a target hole on a suspended SiN membrane with 1m precision via a site-specific transfer-printing method .
	manualset3
148688	1	407640	13	NULL	NULL	NULL	NULL	Aspergillus isolation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A possible new pathogenic Aspergillus isolation and general mycological properties of the fungus .
	manualset3
148689	2	407640	13	NULL	NULL	0	NULL	mycological properties	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A possible new pathogenic Aspergillus isolation and general mycological properties of the fungus .
	manualset3
148690	3	407640	13	NULL	NULL	0	NULL	fungus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A possible new pathogenic Aspergillus isolation and general mycological properties of the fungus .
	manualset3
148691	1	407641	13	NULL	NULL	0	NULL	antibody assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , the antibody assay for Borrelia burgdorferi was positive and the antimicrobial regime was changed to ceftriaxone .
	manualset3
148692	2	407641	13	NULL	NULL	0	NULL	Borrelia burgdorferi	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , the antibody assay for Borrelia burgdorferi was positive and the antimicrobial regime was changed to ceftriaxone .
	manualset3
148693	3	407641	13	NULL	NULL	0	NULL	antimicrobial regime	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , the antibody assay for Borrelia burgdorferi was positive and the antimicrobial regime was changed to ceftriaxone .
	manualset3
148694	4	407641	13	NULL	NULL	0	NULL	ceftriaxone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , the antibody assay for Borrelia burgdorferi was positive and the antimicrobial regime was changed to ceftriaxone .
	manualset3
148695	1	407642	13	NULL	NULL	0	NULL	phosphorus	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , the dissolved phosphorus is precipitated as calcium phosphate with low heavy metal content and recovered from the alkaline solution .
	manualset3
148696	2	407642	13	NULL	NULL	0	NULL	calcium phosphate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , the dissolved phosphorus is precipitated as calcium phosphate with low heavy metal content and recovered from the alkaline solution .
	manualset3
148697	3	407642	13	NULL	NULL	0	NULL	low heavy metal content	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , the dissolved phosphorus is precipitated as calcium phosphate with low heavy metal content and recovered from the alkaline solution .
	manualset3
148698	4	407642	13	NULL	NULL	0	NULL	alkaline solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , the dissolved phosphorus is precipitated as calcium phosphate with low heavy metal content and recovered from the alkaline solution .
	manualset3
148699	1	407643	13	NULL	NULL	0	NULL	novel assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , these novel assays , a CT RRA and a CT luminescence receptor assay , were compared to the conventional RRA based on porcine antigen in a blinded clinical multicenter trial .
	manualset3
148700	2	407643	13	NULL	NULL	0	NULL	CT RRA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , these novel assays , a CT RRA and a CT luminescence receptor assay , were compared to the conventional RRA based on porcine antigen in a blinded clinical multicenter trial .
	manualset3
148701	3	407643	13	NULL	NULL	0	NULL	CT luminescence receptor assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , these novel assays , a CT RRA and a CT luminescence receptor assay , were compared to the conventional RRA based on porcine antigen in a blinded clinical multicenter trial .
	manualset3
148702	4	407643	13	NULL	NULL	0	NULL	conventional RRA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , these novel assays , a CT RRA and a CT luminescence receptor assay , were compared to the conventional RRA based on porcine antigen in a blinded clinical multicenter trial .
	manualset3
148703	5	407643	13	NULL	NULL	0	NULL	porcine antigen 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , these novel assays , a CT RRA and a CT luminescence receptor assay , were compared to the conventional RRA based on porcine antigen in a blinded clinical multicenter trial .
	manualset3
148704	6	407643	13	NULL	NULL	0	NULL	blinded clinical multicenter trial	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , these novel assays , a CT RRA and a CT luminescence receptor assay , were compared to the conventional RRA based on porcine antigen in a blinded clinical multicenter trial .
	manualset3
148705	1	407644	13	NULL	NULL	0	NULL	CHO cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently a stable CHO cell line expressing the receptor fused at its C-terminal part with the enhanced green fluorescent protein ( EGFP ) was established , allowing to verify its cell surface distribution and to determine the affinity of various apelin and angiotensin fragments on the cloned receptor .
	manualset3
148706	2	407644	13	NULL	NULL	0	NULL	receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently a stable CHO cell line expressing the receptor fused at its C-terminal part with the enhanced green fluorescent protein ( EGFP ) was established , allowing to verify its cell surface distribution and to determine the affinity of various apelin and angiotensin fragments on the cloned receptor .
	manualset3
148707	3	407644	13	NULL	NULL	0	NULL	C-terminal part	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently a stable CHO cell line expressing the receptor fused at its C-terminal part with the enhanced green fluorescent protein ( EGFP ) was established , allowing to verify its cell surface distribution and to determine the affinity of various apelin and angiotensin fragments on the cloned receptor .
	manualset3
148708	4	407644	13	NULL	NULL	0	NULL	enhanced green fluorescent protein ( EGFP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently a stable CHO cell line expressing the receptor fused at its C-terminal part with the enhanced green fluorescent protein ( EGFP ) was established , allowing to verify its cell surface distribution and to determine the affinity of various apelin and angiotensin fragments on the cloned receptor .
	manualset3
148709	5	407644	13	NULL	NULL	0	NULL	cell surface distribution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently a stable CHO cell line expressing the receptor fused at its C-terminal part with the enhanced green fluorescent protein ( EGFP ) was established , allowing to verify its cell surface distribution and to determine the affinity of various apelin and angiotensin fragments on the cloned receptor .
	manualset3
148710	6	407644	13	NULL	NULL	0	NULL	affinity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently a stable CHO cell line expressing the receptor fused at its C-terminal part with the enhanced green fluorescent protein ( EGFP ) was established , allowing to verify its cell surface distribution and to determine the affinity of various apelin and angiotensin fragments on the cloned receptor .
	manualset3
148711	7	407644	13	NULL	NULL	0	NULL	apelin 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently a stable CHO cell line expressing the receptor fused at its C-terminal part with the enhanced green fluorescent protein ( EGFP ) was established , allowing to verify its cell surface distribution and to determine the affinity of various apelin and angiotensin fragments on the cloned receptor .
	manualset3
148712	8	407644	13	NULL	NULL	0	NULL	angiotensin fragments	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently a stable CHO cell line expressing the receptor fused at its C-terminal part with the enhanced green fluorescent protein ( EGFP ) was established , allowing to verify its cell surface distribution and to determine the affinity of various apelin and angiotensin fragments on the cloned receptor .
	manualset3
148713	9	407644	13	NULL	NULL	0	NULL	cloned receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently a stable CHO cell line expressing the receptor fused at its C-terminal part with the enhanced green fluorescent protein ( EGFP ) was established , allowing to verify its cell surface distribution and to determine the affinity of various apelin and angiotensin fragments on the cloned receptor .
	manualset3
148714	1	407645	13	NULL	NULL	0	NULL	oxygen consumption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently the oxygen consumption falls to below control levels at older ages .
	manualset3
148715	2	407645	13	NULL	NULL	0	NULL	control levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently the oxygen consumption falls to below control levels at older ages .
	manualset3
148716	3	407645	13	NULL	NULL	0	NULL	older ages	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently the oxygen consumption falls to below control levels at older ages .
	manualset3
148717	1	407646	13	NULL	NULL	NULL	NULL	Substantative local constrictions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Substantative local constrictions to phenylephrine ( PE ) were poorly conducted to the 0.4-mm site in normotensive and hypertensive hamsters .
	manualset3
148718	2	407646	13	NULL	NULL	0	NULL	phenylephrine ( PE )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Substantative local constrictions to phenylephrine ( PE ) were poorly conducted to the 0.4-mm site in normotensive and hypertensive hamsters .
	manualset3
148719	3	407646	13	NULL	NULL	0	NULL	0.4-mm site	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Substantative local constrictions to phenylephrine ( PE ) were poorly conducted to the 0.4-mm site in normotensive and hypertensive hamsters .
	manualset3
148720	4	407646	13	NULL	NULL	0	NULL	normotensive hamsters	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Substantative local constrictions to phenylephrine ( PE ) were poorly conducted to the 0.4-mm site in normotensive and hypertensive hamsters .
	manualset3
148721	5	407646	13	NULL	NULL	0	NULL	hypertensive hamsters	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Substantative local constrictions to phenylephrine ( PE ) were poorly conducted to the 0.4-mm site in normotensive and hypertensive hamsters .
	manualset3
148722	1	407647	13	NULL	NULL	0	NULL	Substantia nigra ( SN ) hyperechogenicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Substantia nigra ( SN ) hyperechogenicity -- a sonographic vulnerability marker for Parkinson 's disease ( PD ) -- has been recently described in patients with idiopathic REM sleep behavior disorder ( RBD ) .
	manualset3
148723	2	407647	13	NULL	NULL	0	NULL	sonographic vulnerability marker	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Substantia nigra ( SN ) hyperechogenicity -- a sonographic vulnerability marker for Parkinson 's disease ( PD ) -- has been recently described in patients with idiopathic REM sleep behavior disorder ( RBD ) .
	manualset3
148724	3	407647	13	NULL	NULL	0	NULL	Parkinson 's disease ( PD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Substantia nigra ( SN ) hyperechogenicity -- a sonographic vulnerability marker for Parkinson 's disease ( PD ) -- has been recently described in patients with idiopathic REM sleep behavior disorder ( RBD ) .
	manualset3
148725	4	407647	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Substantia nigra ( SN ) hyperechogenicity -- a sonographic vulnerability marker for Parkinson 's disease ( PD ) -- has been recently described in patients with idiopathic REM sleep behavior disorder ( RBD ) .
	manualset3
148726	5	407647	13	NULL	NULL	0	NULL	idiopathic REM sleep behavior disorder ( RBD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Substantia nigra ( SN ) hyperechogenicity -- a sonographic vulnerability marker for Parkinson 's disease ( PD ) -- has been recently described in patients with idiopathic REM sleep behavior disorder ( RBD ) .
	manualset3
148727	1	407648	13	NULL	NULL	0	NULL	Substitutes	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitutes for red cell transfusion : 2000-2015 A.D .
	manualset3
148728	2	407648	13	NULL	NULL	0	NULL	red cell transfusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitutes for red cell transfusion : 2000-2015 A.D .
	manualset3
148729	3	407648	13	NULL	NULL	0	NULL	2000-2015 A.D	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitutes for red cell transfusion : 2000-2015 A.D .
	manualset3
148730	1	407649	13	NULL	NULL	0	NULL	Substitution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitution of a less hydrophobic residue into the peptide chain led to a decrease in or even loss of detectable activity , although such peptides retained the immunosuppressive properties .
	manualset3
148731	2	407649	13	NULL	NULL	0	NULL	hydrophobic residue	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitution of a less hydrophobic residue into the peptide chain led to a decrease in or even loss of detectable activity , although such peptides retained the immunosuppressive properties .
	manualset3
148732	3	407649	13	NULL	NULL	0	NULL	peptide chain 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitution of a less hydrophobic residue into the peptide chain led to a decrease in or even loss of detectable activity , although such peptides retained the immunosuppressive properties .
	manualset3
148733	4	407649	13	NULL	NULL	0	NULL	decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitution of a less hydrophobic residue into the peptide chain led to a decrease in or even loss of detectable activity , although such peptides retained the immunosuppressive properties .
	manualset3
148734	5	407649	13	NULL	NULL	0	NULL	loss	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitution of a less hydrophobic residue into the peptide chain led to a decrease in or even loss of detectable activity , although such peptides retained the immunosuppressive properties .
	manualset3
148735	6	407649	13	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitution of a less hydrophobic residue into the peptide chain led to a decrease in or even loss of detectable activity , although such peptides retained the immunosuppressive properties .
	manualset3
148736	7	407649	13	NULL	NULL	0	NULL	peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitution of a less hydrophobic residue into the peptide chain led to a decrease in or even loss of detectable activity , although such peptides retained the immunosuppressive properties .
	manualset3
148737	8	407649	13	NULL	NULL	0	NULL	immunosuppressive properties	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitution of a less hydrophobic residue into the peptide chain led to a decrease in or even loss of detectable activity , although such peptides retained the immunosuppressive properties .
	manualset3
148738	1	407650	13	NULL	NULL	0	NULL	Substitution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitution within the same category , such as from valine to alanine or cysteine among the aliphatic hydrophobic residues , has little effect on association rates with the elastolytic enzymes tested .
	manualset3
148739	2	407650	13	NULL	NULL	0	NULL	category	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitution within the same category , such as from valine to alanine or cysteine among the aliphatic hydrophobic residues , has little effect on association rates with the elastolytic enzymes tested .
	manualset3
148740	3	407650	13	NULL	NULL	0	NULL	valine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitution within the same category , such as from valine to alanine or cysteine among the aliphatic hydrophobic residues , has little effect on association rates with the elastolytic enzymes tested .
	manualset3
148741	4	407650	13	NULL	NULL	0	NULL	alanine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitution within the same category , such as from valine to alanine or cysteine among the aliphatic hydrophobic residues , has little effect on association rates with the elastolytic enzymes tested .
	manualset3
148742	5	407650	13	NULL	NULL	0	NULL	cysteine 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitution within the same category , such as from valine to alanine or cysteine among the aliphatic hydrophobic residues , has little effect on association rates with the elastolytic enzymes tested .
	manualset3
148743	6	407650	13	NULL	NULL	0	NULL	aliphatic hydrophobic residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitution within the same category , such as from valine to alanine or cysteine among the aliphatic hydrophobic residues , has little effect on association rates with the elastolytic enzymes tested .
	manualset3
148744	7	407650	13	NULL	NULL	0	NULL	association rates	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitution within the same category , such as from valine to alanine or cysteine among the aliphatic hydrophobic residues , has little effect on association rates with the elastolytic enzymes tested .
	manualset3
148745	8	407650	13	NULL	NULL	0	NULL	elastolytic enzymes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitution within the same category , such as from valine to alanine or cysteine among the aliphatic hydrophobic residues , has little effect on association rates with the elastolytic enzymes tested .
	manualset3
148746	9	407650	13	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitution within the same category , such as from valine to alanine or cysteine among the aliphatic hydrophobic residues , has little effect on association rates with the elastolytic enzymes tested .
	manualset3
148747	1	407651	13	NULL	NULL	0	NULL	Substitutions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitutions classically associated with resistance to antiretroviral drugs were observed in six of seven samples , including G48V , V82A , L90M , M46I in the protease protein , and K70R , D69D/N , M184V , T215F , K103N in the reverse transcriptase protein .
	manualset3
148748	2	407651	13	NULL	NULL	0	NULL	resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitutions classically associated with resistance to antiretroviral drugs were observed in six of seven samples , including G48V , V82A , L90M , M46I in the protease protein , and K70R , D69D/N , M184V , T215F , K103N in the reverse transcriptase protein .
	manualset3
148749	3	407651	13	NULL	NULL	0	NULL	antiretroviral drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitutions classically associated with resistance to antiretroviral drugs were observed in six of seven samples , including G48V , V82A , L90M , M46I in the protease protein , and K70R , D69D/N , M184V , T215F , K103N in the reverse transcriptase protein .
	manualset3
148750	4	407651	13	NULL	NULL	0	NULL	six of seven samples	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitutions classically associated with resistance to antiretroviral drugs were observed in six of seven samples , including G48V , V82A , L90M , M46I in the protease protein , and K70R , D69D/N , M184V , T215F , K103N in the reverse transcriptase protein .
	manualset3
148751	5	407651	13	NULL	NULL	0	NULL	G48V 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitutions classically associated with resistance to antiretroviral drugs were observed in six of seven samples , including G48V , V82A , L90M , M46I in the protease protein , and K70R , D69D/N , M184V , T215F , K103N in the reverse transcriptase protein .
	manualset3
148752	6	407651	13	NULL	NULL	0	NULL	V82A	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitutions classically associated with resistance to antiretroviral drugs were observed in six of seven samples , including G48V , V82A , L90M , M46I in the protease protein , and K70R , D69D/N , M184V , T215F , K103N in the reverse transcriptase protein .
	manualset3
148753	7	407651	13	NULL	NULL	0	NULL	L90M	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitutions classically associated with resistance to antiretroviral drugs were observed in six of seven samples , including G48V , V82A , L90M , M46I in the protease protein , and K70R , D69D/N , M184V , T215F , K103N in the reverse transcriptase protein .
	manualset3
148754	8	407651	13	NULL	NULL	0	NULL	M46I	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitutions classically associated with resistance to antiretroviral drugs were observed in six of seven samples , including G48V , V82A , L90M , M46I in the protease protein , and K70R , D69D/N , M184V , T215F , K103N in the reverse transcriptase protein .
	manualset3
148755	9	407651	13	NULL	NULL	0	NULL	protease protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitutions classically associated with resistance to antiretroviral drugs were observed in six of seven samples , including G48V , V82A , L90M , M46I in the protease protein , and K70R , D69D/N , M184V , T215F , K103N in the reverse transcriptase protein .
	manualset3
148756	10	407651	13	NULL	NULL	0	NULL	K70R	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitutions classically associated with resistance to antiretroviral drugs were observed in six of seven samples , including G48V , V82A , L90M , M46I in the protease protein , and K70R , D69D/N , M184V , T215F , K103N in the reverse transcriptase protein .
	manualset3
148757	11	407651	13	NULL	NULL	0	NULL	D69D/N	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitutions classically associated with resistance to antiretroviral drugs were observed in six of seven samples , including G48V , V82A , L90M , M46I in the protease protein , and K70R , D69D/N , M184V , T215F , K103N in the reverse transcriptase protein .
	manualset3
148758	12	407651	13	NULL	NULL	0	NULL	M184V	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitutions classically associated with resistance to antiretroviral drugs were observed in six of seven samples , including G48V , V82A , L90M , M46I in the protease protein , and K70R , D69D/N , M184V , T215F , K103N in the reverse transcriptase protein .
	manualset3
148759	13	407651	13	NULL	NULL	0	NULL	T215F	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitutions classically associated with resistance to antiretroviral drugs were observed in six of seven samples , including G48V , V82A , L90M , M46I in the protease protein , and K70R , D69D/N , M184V , T215F , K103N in the reverse transcriptase protein .
	manualset3
148760	14	407651	13	NULL	NULL	0	NULL	K103N	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitutions classically associated with resistance to antiretroviral drugs were observed in six of seven samples , including G48V , V82A , L90M , M46I in the protease protein , and K70R , D69D/N , M184V , T215F , K103N in the reverse transcriptase protein .
	manualset3
148761	15	407651	13	NULL	NULL	0	NULL	reverse transcriptase protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Substitutions classically associated with resistance to antiretroviral drugs were observed in six of seven samples , including G48V , V82A , L90M , M46I in the protease protein , and K70R , D69D/N , M184V , T215F , K103N in the reverse transcriptase protein .
	manualset3
148762	1	407652	13	NULL	NULL	0	NULL	Substrate-induced conformational changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Substrate-induced conformational changes of extracellular loop 1 in the glycine transporter GLYT2 .
	manualset3
148763	2	407652	13	NULL	NULL	0	NULL	extracellular loop 1	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Substrate-induced conformational changes of extracellular loop 1 in the glycine transporter GLYT2 .
	manualset3
148764	3	407652	13	NULL	NULL	0	NULL	glycine transporter GLYT2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Substrate-induced conformational changes of extracellular loop 1 in the glycine transporter GLYT2 .
	manualset3
148765	1	407653	13	NULL	NULL	0	NULL	Substrate 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Substrate was delivered from the organic phase to aqueous phase containing cholesterol oxidase and the product formed partitions back to the organic phase .
	manualset3
148766	2	407653	13	NULL	NULL	0	NULL	organic phase 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Substrate was delivered from the organic phase to aqueous phase containing cholesterol oxidase and the product formed partitions back to the organic phase .
	manualset3
148767	3	407653	13	NULL	NULL	0	NULL	aqueous phase	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Substrate was delivered from the organic phase to aqueous phase containing cholesterol oxidase and the product formed partitions back to the organic phase .
	manualset3
148768	4	407653	13	NULL	NULL	0	NULL	cholesterol oxidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Substrate was delivered from the organic phase to aqueous phase containing cholesterol oxidase and the product formed partitions back to the organic phase .
	manualset3
148769	5	407653	13	NULL	NULL	0	NULL	product 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Substrate was delivered from the organic phase to aqueous phase containing cholesterol oxidase and the product formed partitions back to the organic phase .
	manualset3
148770	6	407653	13	NULL	NULL	0	NULL	partitions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Substrate was delivered from the organic phase to aqueous phase containing cholesterol oxidase and the product formed partitions back to the organic phase .
	manualset3
148771	7	407653	13	NULL	NULL	0	NULL	organic phase 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Substrate was delivered from the organic phase to aqueous phase containing cholesterol oxidase and the product formed partitions back to the organic phase .
	manualset3
148772	1	407654	13	NULL	NULL	0	NULL	Substrates	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Substrates studied included short-chain , medium-chain , and long-chain fructooligosaccharides , oligofructose-enriched inulin , galactooligosaccharide , and polydextrose .
	manualset3
148773	2	407654	13	NULL	NULL	0	NULL	short-chain fructooligosaccharides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Substrates studied included short-chain , medium-chain , and long-chain fructooligosaccharides , oligofructose-enriched inulin , galactooligosaccharide , and polydextrose .
	manualset3
148774	3	407654	13	NULL	NULL	0	NULL	medium-chain fructooligosaccharides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Substrates studied included short-chain , medium-chain , and long-chain fructooligosaccharides , oligofructose-enriched inulin , galactooligosaccharide , and polydextrose .
	manualset3
148775	4	407654	13	NULL	NULL	0	NULL	long-chain fructooligosaccharides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Substrates studied included short-chain , medium-chain , and long-chain fructooligosaccharides , oligofructose-enriched inulin , galactooligosaccharide , and polydextrose .
	manualset3
148776	5	407654	13	NULL	NULL	0	NULL	oligofructose-enriched inulin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Substrates studied included short-chain , medium-chain , and long-chain fructooligosaccharides , oligofructose-enriched inulin , galactooligosaccharide , and polydextrose .
	manualset3
148777	6	407654	13	NULL	NULL	0	NULL	galactooligosaccharide	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Substrates studied included short-chain , medium-chain , and long-chain fructooligosaccharides , oligofructose-enriched inulin , galactooligosaccharide , and polydextrose .
	manualset3
148778	7	407654	13	NULL	NULL	0	NULL	polydextrose	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Substrates studied included short-chain , medium-chain , and long-chain fructooligosaccharides , oligofructose-enriched inulin , galactooligosaccharide , and polydextrose .
	manualset3
148779	1	407655	13	NULL	NULL	0	NULL	Subthalamo-pallido-striatal axis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subthalamo-pallido-striatal axis : a feedback system in the basal ganglia .
	manualset3
148780	2	407655	13	NULL	NULL	0	NULL	feedback system 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subthalamo-pallido-striatal axis : a feedback system in the basal ganglia .
	manualset3
148781	3	407655	13	NULL	NULL	0	NULL	basal ganglia	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Subthalamo-pallido-striatal axis : a feedback system in the basal ganglia .
	manualset3
148782	1	407656	13	NULL	NULL	0	NULL	Success	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Success in cloning the remaining adenosine transporter genes will improve our understanding of the diversity of nucleoside transport processes , with a view to better targeting of therapeutic nucleoside analogs and protective use of transport inhibitors .
	manualset3
148783	2	407656	13	NULL	NULL	0	NULL	adenosine transporter genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Success in cloning the remaining adenosine transporter genes will improve our understanding of the diversity of nucleoside transport processes , with a view to better targeting of therapeutic nucleoside analogs and protective use of transport inhibitors .
	manualset3
148784	3	407656	13	NULL	NULL	0	NULL	understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Success in cloning the remaining adenosine transporter genes will improve our understanding of the diversity of nucleoside transport processes , with a view to better targeting of therapeutic nucleoside analogs and protective use of transport inhibitors .
	manualset3
148785	4	407656	13	NULL	NULL	0	NULL	diversity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Success in cloning the remaining adenosine transporter genes will improve our understanding of the diversity of nucleoside transport processes , with a view to better targeting of therapeutic nucleoside analogs and protective use of transport inhibitors .
	manualset3
148786	5	407656	13	NULL	NULL	0	NULL	 nucleoside transport processes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Success in cloning the remaining adenosine transporter genes will improve our understanding of the diversity of nucleoside transport processes , with a view to better targeting of therapeutic nucleoside analogs and protective use of transport inhibitors .
	manualset3
148787	6	407656	13	NULL	NULL	0	NULL	view	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Success in cloning the remaining adenosine transporter genes will improve our understanding of the diversity of nucleoside transport processes , with a view to better targeting of therapeutic nucleoside analogs and protective use of transport inhibitors .
	manualset3
148788	7	407656	13	NULL	NULL	0	NULL	therapeutic nucleoside analogs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Success in cloning the remaining adenosine transporter genes will improve our understanding of the diversity of nucleoside transport processes , with a view to better targeting of therapeutic nucleoside analogs and protective use of transport inhibitors .
	manualset3
148789	8	407656	13	NULL	NULL	0	NULL	transport inhibitors 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Success in cloning the remaining adenosine transporter genes will improve our understanding of the diversity of nucleoside transport processes , with a view to better targeting of therapeutic nucleoside analogs and protective use of transport inhibitors .
	manualset3
148790	1	407657	13	NULL	NULL	0	NULL	source	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A possible source of the release of PG in the present study was discussed .
	manualset3
148791	2	407657	13	NULL	NULL	0	NULL	release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A possible source of the release of PG in the present study was discussed .
	manualset3
148792	3	407657	13	NULL	NULL	0	NULL	PG 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A possible source of the release of PG in the present study was discussed .
	manualset3
148793	4	407657	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A possible source of the release of PG in the present study was discussed .
	manualset3
148794	1	407658	13	NULL	NULL	0	NULL	Success	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Success in using osseointegrated dental implants-optimal function , esthetics , and phonetics-requires selection of the treatment modality that is optimal for the patient , protection of tissue blood supply , and adherence to a plan based on a thorough analysis of all deviations from the normal anatomy .
	manualset3
148795	2	407658	13	NULL	NULL	0	NULL	dental implants-optimal function 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Success in using osseointegrated dental implants-optimal function , esthetics , and phonetics-requires selection of the treatment modality that is optimal for the patient , protection of tissue blood supply , and adherence to a plan based on a thorough analysis of all deviations from the normal anatomy .
	manualset3
148796	3	407658	13	NULL	NULL	0	NULL	esthetics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Success in using osseointegrated dental implants-optimal function , esthetics , and phonetics-requires selection of the treatment modality that is optimal for the patient , protection of tissue blood supply , and adherence to a plan based on a thorough analysis of all deviations from the normal anatomy .
	manualset3
148797	4	407658	13	NULL	NULL	0	NULL	phonetics-requires selection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Success in using osseointegrated dental implants-optimal function , esthetics , and phonetics-requires selection of the treatment modality that is optimal for the patient , protection of tissue blood supply , and adherence to a plan based on a thorough analysis of all deviations from the normal anatomy .
	manualset3
148798	5	407658	13	NULL	NULL	0	NULL	treatment modality	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Success in using osseointegrated dental implants-optimal function , esthetics , and phonetics-requires selection of the treatment modality that is optimal for the patient , protection of tissue blood supply , and adherence to a plan based on a thorough analysis of all deviations from the normal anatomy .
	manualset3
148799	6	407658	13	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Success in using osseointegrated dental implants-optimal function , esthetics , and phonetics-requires selection of the treatment modality that is optimal for the patient , protection of tissue blood supply , and adherence to a plan based on a thorough analysis of all deviations from the normal anatomy .
	manualset3
148800	7	407658	13	NULL	NULL	0	NULL	protection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Success in using osseointegrated dental implants-optimal function , esthetics , and phonetics-requires selection of the treatment modality that is optimal for the patient , protection of tissue blood supply , and adherence to a plan based on a thorough analysis of all deviations from the normal anatomy .
	manualset3
148801	8	407658	13	NULL	NULL	0	NULL	tissue blood supply	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Success in using osseointegrated dental implants-optimal function , esthetics , and phonetics-requires selection of the treatment modality that is optimal for the patient , protection of tissue blood supply , and adherence to a plan based on a thorough analysis of all deviations from the normal anatomy .
	manualset3
148802	9	407658	13	NULL	NULL	0	NULL	adherence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Success in using osseointegrated dental implants-optimal function , esthetics , and phonetics-requires selection of the treatment modality that is optimal for the patient , protection of tissue blood supply , and adherence to a plan based on a thorough analysis of all deviations from the normal anatomy .
	manualset3
148803	10	407658	13	NULL	NULL	0	NULL	plan	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Success in using osseointegrated dental implants-optimal function , esthetics , and phonetics-requires selection of the treatment modality that is optimal for the patient , protection of tissue blood supply , and adherence to a plan based on a thorough analysis of all deviations from the normal anatomy .
	manualset3
148804	11	407658	13	NULL	NULL	0	NULL	thorough analysis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Success in using osseointegrated dental implants-optimal function , esthetics , and phonetics-requires selection of the treatment modality that is optimal for the patient , protection of tissue blood supply , and adherence to a plan based on a thorough analysis of all deviations from the normal anatomy .
	manualset3
148805	12	407658	13	NULL	NULL	0	NULL	deviations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Success in using osseointegrated dental implants-optimal function , esthetics , and phonetics-requires selection of the treatment modality that is optimal for the patient , protection of tissue blood supply , and adherence to a plan based on a thorough analysis of all deviations from the normal anatomy .
	manualset3
148806	13	407658	13	NULL	NULL	0	NULL	normal anatomy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Success in using osseointegrated dental implants-optimal function , esthetics , and phonetics-requires selection of the treatment modality that is optimal for the patient , protection of tissue blood supply , and adherence to a plan based on a thorough analysis of all deviations from the normal anatomy .
	manualset3
148807	1	407659	13	NULL	NULL	0	NULL	 laparoscopic cholecystectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful laparoscopic cholecystectomy in the third trimester of pregnancy .
	manualset3
148808	2	407659	13	NULL	NULL	0	NULL	third trimester of pregnancy	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful laparoscopic cholecystectomy in the third trimester of pregnancy .
	manualset3
148809	1	407660	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful treatment can be facilitated by first establishing treatment goals , which include managing acute anxiety and following through to remission .
	manualset3
148810	2	407660	13	NULL	NULL	0	NULL	treatment goals 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful treatment can be facilitated by first establishing treatment goals , which include managing acute anxiety and following through to remission .
	manualset3
148811	3	407660	13	NULL	NULL	0	NULL	anxiety	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful treatment can be facilitated by first establishing treatment goals , which include managing acute anxiety and following through to remission .
	manualset3
151651	4	407660	13	NULL	NULL	0	NULL	remission	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful treatment can be facilitated by first establishing treatment goals , which include managing acute anxiety and following through to remission .
	manualset3
148812	1	407661	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful treatment of anorexia with a combination of high-dose olanzapine , fluoxetine and mirtazapine .
	manualset3
148813	2	407661	13	NULL	NULL	0	NULL	anorexia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful treatment of anorexia with a combination of high-dose olanzapine , fluoxetine and mirtazapine .
	manualset3
148814	3	407661	13	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful treatment of anorexia with a combination of high-dose olanzapine , fluoxetine and mirtazapine .
	manualset3
148815	4	407661	13	NULL	NULL	0	NULL	olanzapine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful treatment of anorexia with a combination of high-dose olanzapine , fluoxetine and mirtazapine .
	manualset3
148816	5	407661	13	NULL	NULL	0	NULL	fluoxetine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful treatment of anorexia with a combination of high-dose olanzapine , fluoxetine and mirtazapine .
	manualset3
148817	6	407661	13	NULL	NULL	0	NULL	mirtazapine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful treatment of anorexia with a combination of high-dose olanzapine , fluoxetine and mirtazapine .
	manualset3
148818	1	407662	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful treatment of giggle incontinence with methylphenidate .
	manualset3
148819	2	407662	13	NULL	NULL	0	NULL	giggle incontinence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful treatment of giggle incontinence with methylphenidate .
	manualset3
148820	3	407662	13	NULL	NULL	0	NULL	methylphenidate	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful treatment of giggle incontinence with methylphenidate .
	manualset3
148821	1	407663	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful treatment of type 1 diabetes and seizures with combined ketogenic diet and insulin .
	manualset3
148822	2	407663	13	NULL	NULL	0	NULL	type 1 diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful treatment of type 1 diabetes and seizures with combined ketogenic diet and insulin .
	manualset3
148823	3	407663	13	NULL	NULL	0	NULL	seizures	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful treatment of type 1 diabetes and seizures with combined ketogenic diet and insulin .
	manualset3
148824	4	407663	13	NULL	NULL	NULL	NULL	ketogenic diet 	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Successful treatment of type 1 diabetes and seizures with combined ketogenic diet and insulin .
	manualset3
148825	5	407663	13	NULL	NULL	0	NULL	insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful treatment of type 1 diabetes and seizures with combined ketogenic diet and insulin .
	manualset3
148826	1	407664	13	NULL	NULL	0	NULL	trimethoprim-sulfamethoxazole therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful trimethoprim-sulfamethoxazole therapy in a patient with hyperimmunoglobulin E syndrome .
	manualset3
148827	2	407664	13	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful trimethoprim-sulfamethoxazole therapy in a patient with hyperimmunoglobulin E syndrome .
	manualset3
148828	3	407664	13	NULL	NULL	0	NULL	hyperimmunoglobulin E syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful trimethoprim-sulfamethoxazole therapy in a patient with hyperimmunoglobulin E syndrome .
	manualset3
148829	1	407665	13	NULL	NULL	0	NULL	biliary accessories	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful use of biliary accessories in antegrade dilation of complex upper esophageal stricture due to chemoradiation and surgery .
	manualset3
148830	2	407665	13	NULL	NULL	0	NULL	antegrade dilation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful use of biliary accessories in antegrade dilation of complex upper esophageal stricture due to chemoradiation and surgery .
	manualset3
148831	3	407665	13	NULL	NULL	0	NULL	upper esophageal stricture 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful use of biliary accessories in antegrade dilation of complex upper esophageal stricture due to chemoradiation and surgery .
	manualset3
148832	4	407665	13	NULL	NULL	0	NULL	chemoradiation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful use of biliary accessories in antegrade dilation of complex upper esophageal stricture due to chemoradiation and surgery .
	manualset3
148833	5	407665	13	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful use of biliary accessories in antegrade dilation of complex upper esophageal stricture due to chemoradiation and surgery .
	manualset3
148834	1	407666	13	NULL	NULL	0	NULL	sedative -- hypnotic agent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A potent , new , sedative -- hypnotic agent : 5 , 7-dihydro-5 , 5 , 7 , 7 - tetramethyl-3 - ( 3-nitrophenyl ) furo ( 3 , 4-e ) - as-triazine 4-oxide .
	manualset3
148835	2	407666	13	NULL	NULL	0	NULL	5 , 7-dihydro-5 , 5 , 7 , 7 - tetramethyl-3 - ( 3-nitrophenyl ) furo ( 3 , 4-e ) - as-triazine 4-oxide 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A potent , new , sedative -- hypnotic agent : 5 , 7-dihydro-5 , 5 , 7 , 7 - tetramethyl-3 - ( 3-nitrophenyl ) furo ( 3 , 4-e ) - as-triazine 4-oxide .
	manualset3
148836	1	407667	13	NULL	NULL	0	NULL	use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful use of isotretinoin in a patient on cyclosporine : apparent lack of toxicity .
	manualset3
148837	2	407667	13	NULL	NULL	0	NULL	isotretinoin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful use of isotretinoin in a patient on cyclosporine : apparent lack of toxicity .
	manualset3
148838	3	407667	13	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful use of isotretinoin in a patient on cyclosporine : apparent lack of toxicity .
	manualset3
148839	4	407667	13	NULL	NULL	0	NULL	cyclosporine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful use of isotretinoin in a patient on cyclosporine : apparent lack of toxicity .
	manualset3
148840	5	407667	13	NULL	NULL	0	NULL	lack of toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Successful use of isotretinoin in a patient on cyclosporine : apparent lack of toxicity .
	manualset3
148841	1	407668	13	NULL	NULL	0	NULL	adipocytokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Such adipocytokines as leptin , resistin , adiponectin and proinflammatory cytokines such as IL-6 , IL-1 , IL-8 , TNF-alpha , IL-18 and hsCRP modulate inflammatory process and lead to damage of joint cartilage .
	manualset3
148842	2	407668	13	NULL	NULL	0	NULL	leptin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Such adipocytokines as leptin , resistin , adiponectin and proinflammatory cytokines such as IL-6 , IL-1 , IL-8 , TNF-alpha , IL-18 and hsCRP modulate inflammatory process and lead to damage of joint cartilage .
	manualset3
148843	3	407668	13	NULL	NULL	0	NULL	resistin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Such adipocytokines as leptin , resistin , adiponectin and proinflammatory cytokines such as IL-6 , IL-1 , IL-8 , TNF-alpha , IL-18 and hsCRP modulate inflammatory process and lead to damage of joint cartilage .
	manualset3
148844	4	407668	13	NULL	NULL	0	NULL	adiponectin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Such adipocytokines as leptin , resistin , adiponectin and proinflammatory cytokines such as IL-6 , IL-1 , IL-8 , TNF-alpha , IL-18 and hsCRP modulate inflammatory process and lead to damage of joint cartilage .
	manualset3
148845	5	407668	13	NULL	NULL	0	NULL	proinflammatory cytokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Such adipocytokines as leptin , resistin , adiponectin and proinflammatory cytokines such as IL-6 , IL-1 , IL-8 , TNF-alpha , IL-18 and hsCRP modulate inflammatory process and lead to damage of joint cartilage .
	manualset3
148846	6	407668	13	NULL	NULL	0	NULL	IL-6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Such adipocytokines as leptin , resistin , adiponectin and proinflammatory cytokines such as IL-6 , IL-1 , IL-8 , TNF-alpha , IL-18 and hsCRP modulate inflammatory process and lead to damage of joint cartilage .
	manualset3
148847	7	407668	13	NULL	NULL	0	NULL	IL-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Such adipocytokines as leptin , resistin , adiponectin and proinflammatory cytokines such as IL-6 , IL-1 , IL-8 , TNF-alpha , IL-18 and hsCRP modulate inflammatory process and lead to damage of joint cartilage .
	manualset3
148848	8	407668	13	NULL	NULL	0	NULL	IL-8 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Such adipocytokines as leptin , resistin , adiponectin and proinflammatory cytokines such as IL-6 , IL-1 , IL-8 , TNF-alpha , IL-18 and hsCRP modulate inflammatory process and lead to damage of joint cartilage .
	manualset3
148849	9	407668	13	NULL	NULL	0	NULL	TNF-alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Such adipocytokines as leptin , resistin , adiponectin and proinflammatory cytokines such as IL-6 , IL-1 , IL-8 , TNF-alpha , IL-18 and hsCRP modulate inflammatory process and lead to damage of joint cartilage .
	manualset3
148850	10	407668	13	NULL	NULL	0	NULL	IL-18	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Such adipocytokines as leptin , resistin , adiponectin and proinflammatory cytokines such as IL-6 , IL-1 , IL-8 , TNF-alpha , IL-18 and hsCRP modulate inflammatory process and lead to damage of joint cartilage .
	manualset3
148851	11	407668	13	NULL	NULL	0	NULL	hsCRP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Such adipocytokines as leptin , resistin , adiponectin and proinflammatory cytokines such as IL-6 , IL-1 , IL-8 , TNF-alpha , IL-18 and hsCRP modulate inflammatory process and lead to damage of joint cartilage .
	manualset3
148853	13	407668	13	NULL	NULL	0	NULL	inflammatory process	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such adipocytokines as leptin , resistin , adiponectin and proinflammatory cytokines such as IL-6 , IL-1 , IL-8 , TNF-alpha , IL-18 and hsCRP modulate inflammatory process and lead to damage of joint cartilage .
	manualset3
148854	14	407668	13	NULL	NULL	0	NULL	damage of joint cartilage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Such adipocytokines as leptin , resistin , adiponectin and proinflammatory cytokines such as IL-6 , IL-1 , IL-8 , TNF-alpha , IL-18 and hsCRP modulate inflammatory process and lead to damage of joint cartilage .
	manualset3
148855	1	407669	13	NULL	NULL	0	NULL	biological rhythms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such biological rhythms have notable periodicity despite the internal and external noise present in each cell .
	manualset3
148856	2	407669	13	NULL	NULL	0	NULL	periodicity 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Such biological rhythms have notable periodicity despite the internal and external noise present in each cell .
	manualset3
148857	3	407669	13	NULL	NULL	0	NULL	internal noise	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such biological rhythms have notable periodicity despite the internal and external noise present in each cell .
	manualset3
148858	4	407669	13	NULL	NULL	0	NULL	external noise	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such biological rhythms have notable periodicity despite the internal and external noise present in each cell .
	manualset3
148859	5	407669	13	NULL	NULL	0	NULL	cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Such biological rhythms have notable periodicity despite the internal and external noise present in each cell .
	manualset3
148860	1	407670	13	NULL	NULL	0	NULL	cultivation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such cultivation is in line with what socioemotional selectivity theory predicts ; specifically , when people age , they become more selective and concentrate on strengthening their relationship with those they are emotionally close to .
	manualset3
148861	2	407670	13	NULL	NULL	0	NULL	socioemotional selectivity theory	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Such cultivation is in line with what socioemotional selectivity theory predicts ; specifically , when people age , they become more selective and concentrate on strengthening their relationship with those they are emotionally close to .
	manualset3
148862	3	407670	13	NULL	NULL	0	NULL	people age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Such cultivation is in line with what socioemotional selectivity theory predicts ; specifically , when people age , they become more selective and concentrate on strengthening their relationship with those they are emotionally close to .
	manualset3
148863	4	407670	13	NULL	NULL	0	NULL	relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Such cultivation is in line with what socioemotional selectivity theory predicts ; specifically , when people age , they become more selective and concentrate on strengthening their relationship with those they are emotionally close to .
	manualset3
148864	1	407671	13	NULL	NULL	0	NULL	positive-strand RNA viruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Such cytoplasmic , positive-strand RNA viruses have a conflict between the processes of translation and negative-strand RNA synthesis , since they occur in opposing directions and utilize positive-strand viral RNA as a template .
	manualset3
148865	2	407671	13	NULL	NULL	NULL	NULL	conflict 	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Such cytoplasmic , positive-strand RNA viruses have a conflict between the processes of translation and negative-strand RNA synthesis , since they occur in opposing directions and utilize positive-strand viral RNA as a template .
	manualset3
148866	3	407671	13	NULL	NULL	0	NULL	processes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such cytoplasmic , positive-strand RNA viruses have a conflict between the processes of translation and negative-strand RNA synthesis , since they occur in opposing directions and utilize positive-strand viral RNA as a template .
	manualset3
148867	4	407671	13	NULL	NULL	0	NULL	translation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such cytoplasmic , positive-strand RNA viruses have a conflict between the processes of translation and negative-strand RNA synthesis , since they occur in opposing directions and utilize positive-strand viral RNA as a template .
	manualset3
148868	5	407671	13	NULL	NULL	0	NULL	negative-strand RNA synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such cytoplasmic , positive-strand RNA viruses have a conflict between the processes of translation and negative-strand RNA synthesis , since they occur in opposing directions and utilize positive-strand viral RNA as a template .
	manualset3
148869	6	407671	13	NULL	NULL	0	NULL	directions	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Such cytoplasmic , positive-strand RNA viruses have a conflict between the processes of translation and negative-strand RNA synthesis , since they occur in opposing directions and utilize positive-strand viral RNA as a template .
	manualset3
148870	7	407671	13	NULL	NULL	0	NULL	positive-strand viral RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Such cytoplasmic , positive-strand RNA viruses have a conflict between the processes of translation and negative-strand RNA synthesis , since they occur in opposing directions and utilize positive-strand viral RNA as a template .
	manualset3
148871	8	407671	13	NULL	NULL	0	NULL	template	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Such cytoplasmic , positive-strand RNA viruses have a conflict between the processes of translation and negative-strand RNA synthesis , since they occur in opposing directions and utilize positive-strand viral RNA as a template .
	manualset3
148872	1	407672	13	NULL	NULL	0	NULL	differences 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Such differences in proportion are unlikely to have occurred by chance ( P & lt ; 0.001 ; chi-square test ) .
	manualset3
148873	2	407672	13	NULL	NULL	NULL	NULL	proportion	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Such differences in proportion are unlikely to have occurred by chance ( P & lt ; 0.001 ; chi-square test ) .
	manualset3
148874	3	407672	13	NULL	NULL	0	NULL	chance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such differences in proportion are unlikely to have occurred by chance ( P & lt ; 0.001 ; chi-square test ) .
	manualset3
148875	4	407672	13	NULL	NULL	0	NULL	P & lt ; 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Such differences in proportion are unlikely to have occurred by chance ( P & lt ; 0.001 ; chi-square test ) .
	manualset3
148876	5	407672	13	NULL	NULL	0	NULL	chi-square test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Such differences in proportion are unlikely to have occurred by chance ( P & lt ; 0.001 ; chi-square test ) .
	manualset3
148877	1	407673	13	NULL	NULL	0	NULL	eco-evolutionary feedbacks	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such eco-evolutionary feedbacks may be a key driver of rates of population growth and range expansion and contraction .
	manualset3
148878	2	407673	13	NULL	NULL	0	NULL	key driver	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such eco-evolutionary feedbacks may be a key driver of rates of population growth and range expansion and contraction .
	manualset3
148879	3	407673	13	NULL	NULL	0	NULL	rates of population growth	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Such eco-evolutionary feedbacks may be a key driver of rates of population growth and range expansion and contraction .
	manualset3
148880	4	407673	13	NULL	NULL	0	NULL	range expansion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such eco-evolutionary feedbacks may be a key driver of rates of population growth and range expansion and contraction .
	manualset3
148881	5	407673	13	NULL	NULL	0	NULL	contraction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such eco-evolutionary feedbacks may be a key driver of rates of population growth and range expansion and contraction .
	manualset3
148882	1	407674	13	NULL	NULL	NULL	NULL	evaluations	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Such evaluations are vital to the optimization of bioreactor culture conditions .
	manualset3
148883	2	407674	13	NULL	NULL	0	NULL	optimization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such evaluations are vital to the optimization of bioreactor culture conditions .
	manualset3
148884	3	407674	13	NULL	NULL	0	NULL	bioreactor culture conditions 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Such evaluations are vital to the optimization of bioreactor culture conditions .
	manualset3
148885	1	407675	13	NULL	NULL	0	NULL	interplay	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such functional interplay between RyR1 and RyR3 can serve important roles in Ca ( 2 + ) signaling of cell differentiation and muscle contraction .
	manualset3
148886	2	407675	13	NULL	NULL	0	NULL	RyR1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Such functional interplay between RyR1 and RyR3 can serve important roles in Ca ( 2 + ) signaling of cell differentiation and muscle contraction .
	manualset3
148887	3	407675	13	NULL	NULL	0	NULL	RyR3 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Such functional interplay between RyR1 and RyR3 can serve important roles in Ca ( 2 + ) signaling of cell differentiation and muscle contraction .
	manualset3
148888	4	407675	13	NULL	NULL	0	NULL	roles 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such functional interplay between RyR1 and RyR3 can serve important roles in Ca ( 2 + ) signaling of cell differentiation and muscle contraction .
	manualset3
148889	5	407675	13	NULL	NULL	0	NULL	Ca ( 2 + ) signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such functional interplay between RyR1 and RyR3 can serve important roles in Ca ( 2 + ) signaling of cell differentiation and muscle contraction .
	manualset3
148890	6	407675	13	NULL	NULL	0	NULL	cell differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such functional interplay between RyR1 and RyR3 can serve important roles in Ca ( 2 + ) signaling of cell differentiation and muscle contraction .
	manualset3
148891	7	407675	13	NULL	NULL	0	NULL	muscle contraction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such functional interplay between RyR1 and RyR3 can serve important roles in Ca ( 2 + ) signaling of cell differentiation and muscle contraction .
	manualset3
148892	1	407676	13	NULL	NULL	0	NULL	function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A potential function of Brn-5 may be to suppress the action of proliferative signals in postmitotic neurons and thus prevents them from reentering the cell cycle .
	manualset3
148893	2	407676	13	NULL	NULL	0	NULL	Brn-5 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A potential function of Brn-5 may be to suppress the action of proliferative signals in postmitotic neurons and thus prevents them from reentering the cell cycle .
	manualset3
148894	3	407676	13	NULL	NULL	NULL	NULL	action	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A potential function of Brn-5 may be to suppress the action of proliferative signals in postmitotic neurons and thus prevents them from reentering the cell cycle .
	manualset3
148895	4	407676	13	NULL	NULL	0	NULL	proliferative signals 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A potential function of Brn-5 may be to suppress the action of proliferative signals in postmitotic neurons and thus prevents them from reentering the cell cycle .
	manualset3
148896	5	407676	13	NULL	NULL	0	NULL	postmitotic neurons 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A potential function of Brn-5 may be to suppress the action of proliferative signals in postmitotic neurons and thus prevents them from reentering the cell cycle .
	manualset3
148897	6	407676	13	NULL	NULL	0	NULL	cell cycle	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A potential function of Brn-5 may be to suppress the action of proliferative signals in postmitotic neurons and thus prevents them from reentering the cell cycle .
	manualset3
148898	1	407677	13	NULL	NULL	0	NULL	issues	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such issues include the location of the health facility , design of the infrastructure , storage of equipment and machines , maintenance , medical , and nonmedical operations .
	manualset3
148899	2	407677	13	NULL	NULL	0	NULL	location	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Such issues include the location of the health facility , design of the infrastructure , storage of equipment and machines , maintenance , medical , and nonmedical operations .
	manualset3
148900	3	407677	13	NULL	NULL	NULL	NULL	health facility 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Such issues include the location of the health facility , design of the infrastructure , storage of equipment and machines , maintenance , medical , and nonmedical operations .
	manualset3
148901	4	407677	13	NULL	NULL	0	NULL	design 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Such issues include the location of the health facility , design of the infrastructure , storage of equipment and machines , maintenance , medical , and nonmedical operations .
	manualset3
148902	5	407677	13	NULL	NULL	0	NULL	infrastructure	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Such issues include the location of the health facility , design of the infrastructure , storage of equipment and machines , maintenance , medical , and nonmedical operations .
	manualset3
148903	6	407677	13	NULL	NULL	0	NULL	storage 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such issues include the location of the health facility , design of the infrastructure , storage of equipment and machines , maintenance , medical , and nonmedical operations .
	manualset3
148904	7	407677	13	NULL	NULL	0	NULL	equipment 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Such issues include the location of the health facility , design of the infrastructure , storage of equipment and machines , maintenance , medical , and nonmedical operations .
	manualset3
148905	8	407677	13	NULL	NULL	0	NULL	machines	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Such issues include the location of the health facility , design of the infrastructure , storage of equipment and machines , maintenance , medical , and nonmedical operations .
	manualset3
148906	9	407677	13	NULL	NULL	0	NULL	maintenance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such issues include the location of the health facility , design of the infrastructure , storage of equipment and machines , maintenance , medical , and nonmedical operations .
	manualset3
148907	10	407677	13	NULL	NULL	0	NULL	medical operations 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Such issues include the location of the health facility , design of the infrastructure , storage of equipment and machines , maintenance , medical , and nonmedical operations .
	manualset3
148908	11	407677	13	NULL	NULL	0	NULL	nonmedical operations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such issues include the location of the health facility , design of the infrastructure , storage of equipment and machines , maintenance , medical , and nonmedical operations .
	manualset3
148909	1	407678	13	NULL	NULL	0	NULL	motor deficits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Such motor deficits in experimental animals can be closely related to loss of striatal dopamine receptors , and similar observations have now been made in humans .
	manualset3
148910	2	407678	13	NULL	NULL	0	NULL	experimental animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Such motor deficits in experimental animals can be closely related to loss of striatal dopamine receptors , and similar observations have now been made in humans .
	manualset3
148911	3	407678	13	NULL	NULL	0	NULL	loss	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such motor deficits in experimental animals can be closely related to loss of striatal dopamine receptors , and similar observations have now been made in humans .
	manualset3
148912	4	407678	13	NULL	NULL	0	NULL	striatal dopamine receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Such motor deficits in experimental animals can be closely related to loss of striatal dopamine receptors , and similar observations have now been made in humans .
	manualset3
148913	5	407678	13	NULL	NULL	0	NULL	observations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such motor deficits in experimental animals can be closely related to loss of striatal dopamine receptors , and similar observations have now been made in humans .
	manualset3
148914	6	407678	13	NULL	NULL	0	NULL	humans	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Such motor deficits in experimental animals can be closely related to loss of striatal dopamine receptors , and similar observations have now been made in humans .
	manualset3
148920	1	407679	13	NULL	NULL	0	NULL	observations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such observations have led to a widespread belief that dietary NaCl is important in hypertensives only if blood pressure changes are observed after changes in NaCl intake .
	manualset3
148921	2	407679	13	NULL	NULL	0	NULL	belief	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such observations have led to a widespread belief that dietary NaCl is important in hypertensives only if blood pressure changes are observed after changes in NaCl intake .
	manualset3
148922	3	407679	13	NULL	NULL	0	NULL	dietary NaCl 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Such observations have led to a widespread belief that dietary NaCl is important in hypertensives only if blood pressure changes are observed after changes in NaCl intake .
	manualset3
148923	4	407679	13	NULL	NULL	0	NULL	hypertensives	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Such observations have led to a widespread belief that dietary NaCl is important in hypertensives only if blood pressure changes are observed after changes in NaCl intake .
	manualset3
148924	5	407679	13	NULL	NULL	0	NULL	blood pressure changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Such observations have led to a widespread belief that dietary NaCl is important in hypertensives only if blood pressure changes are observed after changes in NaCl intake .
	manualset3
148925	6	407679	13	NULL	NULL	0	NULL	changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such observations have led to a widespread belief that dietary NaCl is important in hypertensives only if blood pressure changes are observed after changes in NaCl intake .
	manualset3
148926	7	407679	13	NULL	NULL	0	NULL	NaCl intake	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Such observations have led to a widespread belief that dietary NaCl is important in hypertensives only if blood pressure changes are observed after changes in NaCl intake .
	manualset3
148929	1	407680	13	NULL	NULL	0	NULL	performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such obviously improved performance of g-C ( 3 ) N ( 4 ) - ZnO can be ascribed mainly to the enhancement of electron-hole separations at the interface of ZnO and g-C ( 3 ) N ( 4 ) .
	manualset3
148930	2	407680	13	NULL	NULL	0	NULL	g-C ( 3 ) N ( 4 ) - ZnO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Such obviously improved performance of g-C ( 3 ) N ( 4 ) - ZnO can be ascribed mainly to the enhancement of electron-hole separations at the interface of ZnO and g-C ( 3 ) N ( 4 ) .
	manualset3
148931	3	407680	13	NULL	NULL	0	NULL	enhancement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such obviously improved performance of g-C ( 3 ) N ( 4 ) - ZnO can be ascribed mainly to the enhancement of electron-hole separations at the interface of ZnO and g-C ( 3 ) N ( 4 ) .
	manualset3
148932	4	407680	13	NULL	NULL	0	NULL	electron-hole separations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such obviously improved performance of g-C ( 3 ) N ( 4 ) - ZnO can be ascribed mainly to the enhancement of electron-hole separations at the interface of ZnO and g-C ( 3 ) N ( 4 ) .
	manualset3
148933	5	407680	13	NULL	NULL	0	NULL	interface	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such obviously improved performance of g-C ( 3 ) N ( 4 ) - ZnO can be ascribed mainly to the enhancement of electron-hole separations at the interface of ZnO and g-C ( 3 ) N ( 4 ) .
	manualset3
148934	6	407680	13	NULL	NULL	0	NULL	ZnO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Such obviously improved performance of g-C ( 3 ) N ( 4 ) - ZnO can be ascribed mainly to the enhancement of electron-hole separations at the interface of ZnO and g-C ( 3 ) N ( 4 ) .
	manualset3
148935	7	407680	13	NULL	NULL	0	NULL	g-C ( 3 ) N ( 4 ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Such obviously improved performance of g-C ( 3 ) N ( 4 ) - ZnO can be ascribed mainly to the enhancement of electron-hole separations at the interface of ZnO and g-C ( 3 ) N ( 4 ) .
	manualset3
148938	1	407681	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Such patients may be appropriate for future drug therapies that affect synuclein pathophysiology , in which the development of parkinsonism and/or dementia could be delayed or prevented .
	manualset3
148946	2	407681	13	NULL	NULL	0	NULL	future drug therapies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Such patients may be appropriate for future drug therapies that affect synuclein pathophysiology , in which the development of parkinsonism and/or dementia could be delayed or prevented .
	manualset3
148947	3	407681	13	NULL	NULL	0	NULL	synuclein pathophysiology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Such patients may be appropriate for future drug therapies that affect synuclein pathophysiology , in which the development of parkinsonism and/or dementia could be delayed or prevented .
	manualset3
148948	4	407681	13	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such patients may be appropriate for future drug therapies that affect synuclein pathophysiology , in which the development of parkinsonism and/or dementia could be delayed or prevented .
	manualset3
148949	5	407681	13	NULL	NULL	0	NULL	parkinsonism	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Such patients may be appropriate for future drug therapies that affect synuclein pathophysiology , in which the development of parkinsonism and/or dementia could be delayed or prevented .
	manualset3
148950	6	407681	13	NULL	NULL	0	NULL	dementia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Such patients may be appropriate for future drug therapies that affect synuclein pathophysiology , in which the development of parkinsonism and/or dementia could be delayed or prevented .
	manualset3
148951	1	407682	13	NULL	NULL	NULL	NULL	procedures	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Such procedures may be useful for controlled and parametric studies of the mobilization of pituitary or brain pools of beta-endorphin under conditions involving merely anticipation of pain rather than the actual activation of ascending nervous pain pathways .
	manualset3
148952	2	407682	13	NULL	NULL	0	NULL	parametric studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Such procedures may be useful for controlled and parametric studies of the mobilization of pituitary or brain pools of beta-endorphin under conditions involving merely anticipation of pain rather than the actual activation of ascending nervous pain pathways .
	manualset3
148953	3	407682	13	NULL	NULL	0	NULL	controlled studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Such procedures may be useful for controlled and parametric studies of the mobilization of pituitary or brain pools of beta-endorphin under conditions involving merely anticipation of pain rather than the actual activation of ascending nervous pain pathways .
	manualset3
148954	4	407682	13	NULL	NULL	0	NULL	mobilization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such procedures may be useful for controlled and parametric studies of the mobilization of pituitary or brain pools of beta-endorphin under conditions involving merely anticipation of pain rather than the actual activation of ascending nervous pain pathways .
	manualset3
148955	5	407682	13	NULL	NULL	0	NULL	pituitary pools	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Such procedures may be useful for controlled and parametric studies of the mobilization of pituitary or brain pools of beta-endorphin under conditions involving merely anticipation of pain rather than the actual activation of ascending nervous pain pathways .
	manualset3
148956	6	407682	13	NULL	NULL	0	NULL	brain pools	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Such procedures may be useful for controlled and parametric studies of the mobilization of pituitary or brain pools of beta-endorphin under conditions involving merely anticipation of pain rather than the actual activation of ascending nervous pain pathways .
	manualset3
148957	7	407682	13	NULL	NULL	0	NULL	beta-endorphin 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Such procedures may be useful for controlled and parametric studies of the mobilization of pituitary or brain pools of beta-endorphin under conditions involving merely anticipation of pain rather than the actual activation of ascending nervous pain pathways .
	manualset3
148958	8	407682	13	NULL	NULL	0	NULL	conditions 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Such procedures may be useful for controlled and parametric studies of the mobilization of pituitary or brain pools of beta-endorphin under conditions involving merely anticipation of pain rather than the actual activation of ascending nervous pain pathways .
	manualset3
148959	9	407682	13	NULL	NULL	0	NULL	anticipation	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such procedures may be useful for controlled and parametric studies of the mobilization of pituitary or brain pools of beta-endorphin under conditions involving merely anticipation of pain rather than the actual activation of ascending nervous pain pathways .
	manualset3
148960	10	407682	13	NULL	NULL	0	NULL	pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Such procedures may be useful for controlled and parametric studies of the mobilization of pituitary or brain pools of beta-endorphin under conditions involving merely anticipation of pain rather than the actual activation of ascending nervous pain pathways .
	manualset3
148961	11	407682	13	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such procedures may be useful for controlled and parametric studies of the mobilization of pituitary or brain pools of beta-endorphin under conditions involving merely anticipation of pain rather than the actual activation of ascending nervous pain pathways .
	manualset3
148962	12	407682	13	NULL	NULL	0	NULL	ascending nervous pain pathways 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such procedures may be useful for controlled and parametric studies of the mobilization of pituitary or brain pools of beta-endorphin under conditions involving merely anticipation of pain rather than the actual activation of ascending nervous pain pathways .
	manualset3
148963	1	407683	13	NULL	NULL	0	NULL	 prophylaxis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Such prophylaxis must be accompanied by risk-reduction counseling , appropriate referrals for treatment , and evaluation for pregnancy and associated sexually transmitted infections .
	manualset3
148964	2	407683	13	NULL	NULL	0	NULL	 risk-reduction counseling	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Such prophylaxis must be accompanied by risk-reduction counseling , appropriate referrals for treatment , and evaluation for pregnancy and associated sexually transmitted infections .
	manualset3
148965	3	407683	13	NULL	NULL	0	NULL	referrals 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such prophylaxis must be accompanied by risk-reduction counseling , appropriate referrals for treatment , and evaluation for pregnancy and associated sexually transmitted infections .
	manualset3
148966	4	407683	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Such prophylaxis must be accompanied by risk-reduction counseling , appropriate referrals for treatment , and evaluation for pregnancy and associated sexually transmitted infections .
	manualset3
148967	5	407683	13	NULL	NULL	0	NULL	evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such prophylaxis must be accompanied by risk-reduction counseling , appropriate referrals for treatment , and evaluation for pregnancy and associated sexually transmitted infections .
	manualset3
148968	6	407683	13	NULL	NULL	0	NULL	pregnancy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such prophylaxis must be accompanied by risk-reduction counseling , appropriate referrals for treatment , and evaluation for pregnancy and associated sexually transmitted infections .
	manualset3
148969	7	407683	13	NULL	NULL	0	NULL	infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Such prophylaxis must be accompanied by risk-reduction counseling , appropriate referrals for treatment , and evaluation for pregnancy and associated sexually transmitted infections .
	manualset3
148971	1	407684	13	NULL	NULL	NULL	NULL	potential risk assessment 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A potential risk assessment of a dengue outbreak in north central Texas , USA .
	manualset3
148972	2	407684	13	NULL	NULL	0	NULL	dengue outbreak 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A potential risk assessment of a dengue outbreak in north central Texas , USA .
	manualset3
148973	3	407684	13	NULL	NULL	0	NULL	north central Texas	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A potential risk assessment of a dengue outbreak in north central Texas , USA .
	manualset3
148974	4	407684	13	NULL	NULL	0	NULL	USA	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A potential risk assessment of a dengue outbreak in north central Texas , USA .
	manualset3
148978	1	407685	13	NULL	NULL	0	NULL	reviews	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such reviews have the potential to identify emerging causes of deaths and associated risk factors , such as ectopic pregnancy deaths among women who use illicit drugs .
	manualset3
148979	2	407685	13	NULL	NULL	0	NULL	causes of deaths	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Such reviews have the potential to identify emerging causes of deaths and associated risk factors , such as ectopic pregnancy deaths among women who use illicit drugs .
	manualset3
148980	3	407685	13	NULL	NULL	0	NULL	risk factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Such reviews have the potential to identify emerging causes of deaths and associated risk factors , such as ectopic pregnancy deaths among women who use illicit drugs .
	manualset3
148981	4	407685	13	NULL	NULL	0	NULL	ectopic pregnancy deaths	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Such reviews have the potential to identify emerging causes of deaths and associated risk factors , such as ectopic pregnancy deaths among women who use illicit drugs .
	manualset3
148982	5	407685	13	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Such reviews have the potential to identify emerging causes of deaths and associated risk factors , such as ectopic pregnancy deaths among women who use illicit drugs .
	manualset3
148983	6	407685	13	NULL	NULL	0	NULL	illicit drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Such reviews have the potential to identify emerging causes of deaths and associated risk factors , such as ectopic pregnancy deaths among women who use illicit drugs .
	manualset3
148984	1	407686	13	NULL	NULL	NULL	NULL	signals	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Such signals , released several millimetres from a growing nerve tip , cause it to change direction and bend towards the source .
	manualset3
148985	2	407686	13	NULL	NULL	0	NULL	millimetres	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Such signals , released several millimetres from a growing nerve tip , cause it to change direction and bend towards the source .
	manualset3
148986	3	407686	13	NULL	NULL	0	NULL	nerve tip 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Such signals , released several millimetres from a growing nerve tip , cause it to change direction and bend towards the source .
	manualset3
148987	4	407686	13	NULL	NULL	0	NULL	cause	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such signals , released several millimetres from a growing nerve tip , cause it to change direction and bend towards the source .
	manualset3
148988	5	407686	13	NULL	NULL	0	NULL	direction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such signals , released several millimetres from a growing nerve tip , cause it to change direction and bend towards the source .
	manualset3
148989	6	407686	13	NULL	NULL	0	NULL	source	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Such signals , released several millimetres from a growing nerve tip , cause it to change direction and bend towards the source .
	manualset3
148990	1	407687	13	NULL	NULL	0	NULL	strategies 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Such strategies , of which several examples are discussed , are cost-effective and lead to improved health in the target population .
	manualset3
148991	2	407687	13	NULL	NULL	0	NULL	examples	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Such strategies , of which several examples are discussed , are cost-effective and lead to improved health in the target population .
	manualset3
148992	3	407687	13	NULL	NULL	0	NULL	health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Such strategies , of which several examples are discussed , are cost-effective and lead to improved health in the target population .
	manualset3
148993	4	407687	13	NULL	NULL	0	NULL	target population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Such strategies , of which several examples are discussed , are cost-effective and lead to improved health in the target population .
	manualset3
148994	1	407688	13	NULL	NULL	0	NULL	stress	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such stress may be increased or decreased , depending on the specific migration experience .
	manualset3
148995	2	407688	13	NULL	NULL	0	NULL	specific migration experience	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such stress may be increased or decreased , depending on the specific migration experience .
	manualset3
148996	1	407689	13	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Such studies initiated by manufacturer are designed to promote product .
	manualset3
148997	2	407689	13	NULL	NULL	0	NULL	manufacturer 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Such studies initiated by manufacturer are designed to promote product .
	manualset3
148998	3	407689	13	NULL	NULL	0	NULL	product 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Such studies initiated by manufacturer are designed to promote product .
	manualset3
148999	1	407690	13	NULL	NULL	0	NULL	work	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Such work is impacted by challenges such as ethical difficulties , professional obstacles , bonding with colleagues and personal issues .
	manualset3
149000	2	407690	13	NULL	NULL	0	NULL	ethical difficulties	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such work is impacted by challenges such as ethical difficulties , professional obstacles , bonding with colleagues and personal issues .
	manualset3
149001	3	407690	13	NULL	NULL	0	NULL	professional obstacles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such work is impacted by challenges such as ethical difficulties , professional obstacles , bonding with colleagues and personal issues .
	manualset3
149002	4	407690	13	NULL	NULL	0	NULL	colleagues 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Such work is impacted by challenges such as ethical difficulties , professional obstacles , bonding with colleagues and personal issues .
	manualset3
149003	5	407690	13	NULL	NULL	0	NULL	personal issues	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such work is impacted by challenges such as ethical difficulties , professional obstacles , bonding with colleagues and personal issues .
	manualset3
149004	1	407691	13	NULL	NULL	0	NULL	mode of binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a mode of binding of inhibitors containing an allophenylnorstatine-dimethylthioproline insert in the P1-P1 ' positions , previously reported in a complex with PMIV , demonstrates the importance of satisfying the requirements for the proper positioning of the functional groups in the mechanism-based inhibitors towards the catalytic machinery of aspartic proteases , as opposed to binding driven solely by the specificity of the individual enzymes .
	manualset3
149005	2	407691	13	NULL	NULL	0	NULL	inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a mode of binding of inhibitors containing an allophenylnorstatine-dimethylthioproline insert in the P1-P1 ' positions , previously reported in a complex with PMIV , demonstrates the importance of satisfying the requirements for the proper positioning of the functional groups in the mechanism-based inhibitors towards the catalytic machinery of aspartic proteases , as opposed to binding driven solely by the specificity of the individual enzymes .
	manualset3
149006	3	407691	13	NULL	NULL	0	NULL	allophenylnorstatine-dimethylthioproline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a mode of binding of inhibitors containing an allophenylnorstatine-dimethylthioproline insert in the P1-P1 ' positions , previously reported in a complex with PMIV , demonstrates the importance of satisfying the requirements for the proper positioning of the functional groups in the mechanism-based inhibitors towards the catalytic machinery of aspartic proteases , as opposed to binding driven solely by the specificity of the individual enzymes .
	manualset3
149007	4	407691	13	NULL	NULL	0	NULL	insert	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a mode of binding of inhibitors containing an allophenylnorstatine-dimethylthioproline insert in the P1-P1 ' positions , previously reported in a complex with PMIV , demonstrates the importance of satisfying the requirements for the proper positioning of the functional groups in the mechanism-based inhibitors towards the catalytic machinery of aspartic proteases , as opposed to binding driven solely by the specificity of the individual enzymes .
	manualset3
149008	5	407691	13	NULL	NULL	0	NULL	P1-P1 ' positions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a mode of binding of inhibitors containing an allophenylnorstatine-dimethylthioproline insert in the P1-P1 ' positions , previously reported in a complex with PMIV , demonstrates the importance of satisfying the requirements for the proper positioning of the functional groups in the mechanism-based inhibitors towards the catalytic machinery of aspartic proteases , as opposed to binding driven solely by the specificity of the individual enzymes .
	manualset3
149009	6	407691	13	NULL	NULL	0	NULL	complex	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a mode of binding of inhibitors containing an allophenylnorstatine-dimethylthioproline insert in the P1-P1 ' positions , previously reported in a complex with PMIV , demonstrates the importance of satisfying the requirements for the proper positioning of the functional groups in the mechanism-based inhibitors towards the catalytic machinery of aspartic proteases , as opposed to binding driven solely by the specificity of the individual enzymes .
	manualset3
149010	7	407691	13	NULL	NULL	0	NULL	PMIV	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a mode of binding of inhibitors containing an allophenylnorstatine-dimethylthioproline insert in the P1-P1 ' positions , previously reported in a complex with PMIV , demonstrates the importance of satisfying the requirements for the proper positioning of the functional groups in the mechanism-based inhibitors towards the catalytic machinery of aspartic proteases , as opposed to binding driven solely by the specificity of the individual enzymes .
	manualset3
149012	8	407691	13	NULL	NULL	0	NULL	importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a mode of binding of inhibitors containing an allophenylnorstatine-dimethylthioproline insert in the P1-P1 ' positions , previously reported in a complex with PMIV , demonstrates the importance of satisfying the requirements for the proper positioning of the functional groups in the mechanism-based inhibitors towards the catalytic machinery of aspartic proteases , as opposed to binding driven solely by the specificity of the individual enzymes .
	manualset3
149013	9	407691	13	NULL	NULL	0	NULL	positioning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a mode of binding of inhibitors containing an allophenylnorstatine-dimethylthioproline insert in the P1-P1 ' positions , previously reported in a complex with PMIV , demonstrates the importance of satisfying the requirements for the proper positioning of the functional groups in the mechanism-based inhibitors towards the catalytic machinery of aspartic proteases , as opposed to binding driven solely by the specificity of the individual enzymes .
	manualset3
149014	10	407691	13	NULL	NULL	0	NULL	functional groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a mode of binding of inhibitors containing an allophenylnorstatine-dimethylthioproline insert in the P1-P1 ' positions , previously reported in a complex with PMIV , demonstrates the importance of satisfying the requirements for the proper positioning of the functional groups in the mechanism-based inhibitors towards the catalytic machinery of aspartic proteases , as opposed to binding driven solely by the specificity of the individual enzymes .
	manualset3
149015	11	407691	13	NULL	NULL	0	NULL	inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a mode of binding of inhibitors containing an allophenylnorstatine-dimethylthioproline insert in the P1-P1 ' positions , previously reported in a complex with PMIV , demonstrates the importance of satisfying the requirements for the proper positioning of the functional groups in the mechanism-based inhibitors towards the catalytic machinery of aspartic proteases , as opposed to binding driven solely by the specificity of the individual enzymes .
	manualset3
149017	12	407691	13	NULL	NULL	0	NULL	catalytic machinery 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a mode of binding of inhibitors containing an allophenylnorstatine-dimethylthioproline insert in the P1-P1 ' positions , previously reported in a complex with PMIV , demonstrates the importance of satisfying the requirements for the proper positioning of the functional groups in the mechanism-based inhibitors towards the catalytic machinery of aspartic proteases , as opposed to binding driven solely by the specificity of the individual enzymes .
	manualset3
149018	13	407691	13	NULL	NULL	0	NULL	aspartic proteases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a mode of binding of inhibitors containing an allophenylnorstatine-dimethylthioproline insert in the P1-P1 ' positions , previously reported in a complex with PMIV , demonstrates the importance of satisfying the requirements for the proper positioning of the functional groups in the mechanism-based inhibitors towards the catalytic machinery of aspartic proteases , as opposed to binding driven solely by the specificity of the individual enzymes .
	manualset3
149019	14	407691	13	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a mode of binding of inhibitors containing an allophenylnorstatine-dimethylthioproline insert in the P1-P1 ' positions , previously reported in a complex with PMIV , demonstrates the importance of satisfying the requirements for the proper positioning of the functional groups in the mechanism-based inhibitors towards the catalytic machinery of aspartic proteases , as opposed to binding driven solely by the specificity of the individual enzymes .
	manualset3
149020	15	407691	13	NULL	NULL	0	NULL	specificity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a mode of binding of inhibitors containing an allophenylnorstatine-dimethylthioproline insert in the P1-P1 ' positions , previously reported in a complex with PMIV , demonstrates the importance of satisfying the requirements for the proper positioning of the functional groups in the mechanism-based inhibitors towards the catalytic machinery of aspartic proteases , as opposed to binding driven solely by the specificity of the individual enzymes .
	manualset3
149021	16	407691	13	NULL	NULL	0	NULL	enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a mode of binding of inhibitors containing an allophenylnorstatine-dimethylthioproline insert in the P1-P1 ' positions , previously reported in a complex with PMIV , demonstrates the importance of satisfying the requirements for the proper positioning of the functional groups in the mechanism-based inhibitors towards the catalytic machinery of aspartic proteases , as opposed to binding driven solely by the specificity of the individual enzymes .
	manualset3
149028	1	407692	13	NULL	NULL	0	NULL	target 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A potential target for the anti-angiogenic action of angiostatin .
	manualset3
149029	2	407692	13	NULL	NULL	0	NULL	anti-angiogenic action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A potential target for the anti-angiogenic action of angiostatin .
	manualset3
149030	3	407692	13	NULL	NULL	0	NULL	angiostatin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A potential target for the anti-angiogenic action of angiostatin .
	manualset3
149042	1	407693	13	NULL	NULL	0	NULL	network	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a network can cope with the problem of vanishing gradient , experienced in prediction with RNN 's .
	manualset3
149043	2	407693	13	NULL	NULL	0	NULL	problem	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a network can cope with the problem of vanishing gradient , experienced in prediction with RNN 's .
	manualset3
149044	3	407693	13	NULL	NULL	0	NULL	vanishing gradient	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a network can cope with the problem of vanishing gradient , experienced in prediction with RNN 's .
	manualset3
149045	4	407693	13	NULL	NULL	0	NULL	prediction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a network can cope with the problem of vanishing gradient , experienced in prediction with RNN 's .
	manualset3
149046	5	407693	13	NULL	NULL	0	NULL	RNN 's	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a network can cope with the problem of vanishing gradient , experienced in prediction with RNN 's .
	manualset3
149049	1	407694	13	NULL	NULL	0	NULL	novel assembly behavior 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a novel assembly behavior indicated a dramatic impact on receptor activation as well as on the signaling mechanism associated with the murine GITRL costimulatory system .
	manualset3
149052	2	407694	13	NULL	NULL	0	NULL	impact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a novel assembly behavior indicated a dramatic impact on receptor activation as well as on the signaling mechanism associated with the murine GITRL costimulatory system .
	manualset3
149053	3	407694	13	NULL	NULL	0	NULL	receptor activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a novel assembly behavior indicated a dramatic impact on receptor activation as well as on the signaling mechanism associated with the murine GITRL costimulatory system .
	manualset3
149054	4	407694	13	NULL	NULL	NULL	NULL	signaling mechanism	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Such a novel assembly behavior indicated a dramatic impact on receptor activation as well as on the signaling mechanism associated with the murine GITRL costimulatory system .
	manualset3
149055	5	407694	13	NULL	NULL	0	NULL	murine GITRL costimulatory system	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a novel assembly behavior indicated a dramatic impact on receptor activation as well as on the signaling mechanism associated with the murine GITRL costimulatory system .
	manualset3
149060	1	407695	13	NULL	NULL	0	NULL	preparation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a preparation deserves further consideration as a possible replacement for digoxin tablets .
	manualset3
149061	2	407695	13	NULL	NULL	0	NULL	consideration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a preparation deserves further consideration as a possible replacement for digoxin tablets .
	manualset3
149062	3	407695	13	NULL	NULL	0	NULL	replacement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a preparation deserves further consideration as a possible replacement for digoxin tablets .
	manualset3
149063	4	407695	13	NULL	NULL	0	NULL	digoxin tablets	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a preparation deserves further consideration as a possible replacement for digoxin tablets .
	manualset3
149064	1	407696	13	NULL	NULL	0	NULL	process	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a process would be adaptive , facilitating fairly fast changes in fetal growth rate as the conditions under which a population lives deteriorate or improve .
	manualset3
149065	2	407696	13	NULL	NULL	0	NULL	changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a process would be adaptive , facilitating fairly fast changes in fetal growth rate as the conditions under which a population lives deteriorate or improve .
	manualset3
149066	3	407696	13	NULL	NULL	0	NULL	fetal growth rate 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a process would be adaptive , facilitating fairly fast changes in fetal growth rate as the conditions under which a population lives deteriorate or improve .
	manualset3
149067	4	407696	13	NULL	NULL	0	NULL	conditions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a process would be adaptive , facilitating fairly fast changes in fetal growth rate as the conditions under which a population lives deteriorate or improve .
	manualset3
149068	5	407696	13	NULL	NULL	0	NULL	population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a process would be adaptive , facilitating fairly fast changes in fetal growth rate as the conditions under which a population lives deteriorate or improve .
	manualset3
149069	6	407696	13	NULL	NULL	0	NULL	lives	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a process would be adaptive , facilitating fairly fast changes in fetal growth rate as the conditions under which a population lives deteriorate or improve .
	manualset3
149070	1	407697	13	NULL	NULL	0	NULL	function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a proposed function for S19 is compatible with its proximity to E131 , the acidic residue in a putative Walker B motif and probable second Mg-ATP ligand in PRK 's active site .
	manualset3
149071	2	407697	13	NULL	NULL	0	NULL	S19	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a proposed function for S19 is compatible with its proximity to E131 , the acidic residue in a putative Walker B motif and probable second Mg-ATP ligand in PRK 's active site .
	manualset3
149072	3	407697	13	NULL	NULL	0	NULL	proximity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a proposed function for S19 is compatible with its proximity to E131 , the acidic residue in a putative Walker B motif and probable second Mg-ATP ligand in PRK 's active site .
	manualset3
149073	4	407697	13	NULL	NULL	0	NULL	E131	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a proposed function for S19 is compatible with its proximity to E131 , the acidic residue in a putative Walker B motif and probable second Mg-ATP ligand in PRK 's active site .
	manualset3
149074	5	407697	13	NULL	NULL	0	NULL	acidic residue	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a proposed function for S19 is compatible with its proximity to E131 , the acidic residue in a putative Walker B motif and probable second Mg-ATP ligand in PRK 's active site .
	manualset3
149075	6	407697	13	NULL	NULL	0	NULL	putative Walker B motif 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a proposed function for S19 is compatible with its proximity to E131 , the acidic residue in a putative Walker B motif and probable second Mg-ATP ligand in PRK 's active site .
	manualset3
149076	7	407697	13	NULL	NULL	0	NULL	second Mg-ATP ligand	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a proposed function for S19 is compatible with its proximity to E131 , the acidic residue in a putative Walker B motif and probable second Mg-ATP ligand in PRK 's active site .
	manualset3
149077	8	407697	13	NULL	NULL	0	NULL	PRK 's active site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a proposed function for S19 is compatible with its proximity to E131 , the acidic residue in a putative Walker B motif and probable second Mg-ATP ligand in PRK 's active site .
	manualset3
149078	1	407698	13	NULL	NULL	0	NULL	technique	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a technique provides an excellent anatomic view , thus avoiding injury to structures in proximity to the hernia during repair ; eventually the well-known advantages of such approach result .
	manualset3
149079	2	407698	13	NULL	NULL	0	NULL	anatomic view	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a technique provides an excellent anatomic view , thus avoiding injury to structures in proximity to the hernia during repair ; eventually the well-known advantages of such approach result .
	manualset3
149080	3	407698	13	NULL	NULL	0	NULL	injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a technique provides an excellent anatomic view , thus avoiding injury to structures in proximity to the hernia during repair ; eventually the well-known advantages of such approach result .
	manualset3
149081	4	407698	13	NULL	NULL	0	NULL	structures	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a technique provides an excellent anatomic view , thus avoiding injury to structures in proximity to the hernia during repair ; eventually the well-known advantages of such approach result .
	manualset3
149082	5	407698	13	NULL	NULL	0	NULL	proximity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a technique provides an excellent anatomic view , thus avoiding injury to structures in proximity to the hernia during repair ; eventually the well-known advantages of such approach result .
	manualset3
149083	6	407698	13	NULL	NULL	0	NULL	hernia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a technique provides an excellent anatomic view , thus avoiding injury to structures in proximity to the hernia during repair ; eventually the well-known advantages of such approach result .
	manualset3
149084	7	407698	13	NULL	NULL	0	NULL	repair	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a technique provides an excellent anatomic view , thus avoiding injury to structures in proximity to the hernia during repair ; eventually the well-known advantages of such approach result .
	manualset3
149085	8	407698	13	NULL	NULL	0	NULL	advantages	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a technique provides an excellent anatomic view , thus avoiding injury to structures in proximity to the hernia during repair ; eventually the well-known advantages of such approach result .
	manualset3
149086	9	407698	13	NULL	NULL	0	NULL	approach result 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a technique provides an excellent anatomic view , thus avoiding injury to structures in proximity to the hernia during repair ; eventually the well-known advantages of such approach result .
	manualset3
149087	1	407699	13	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such an addition also markedly stimulates natural killers of spleen lymphocytes .
	manualset3
149088	2	407699	13	NULL	NULL	0	NULL	natural killers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Such an addition also markedly stimulates natural killers of spleen lymphocytes .
	manualset3
149089	3	407699	13	NULL	NULL	0	NULL	spleen lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Such an addition also markedly stimulates natural killers of spleen lymphocytes .
	manualset3
149090	1	407700	13	NULL	NULL	0	NULL	Sucrose palatability 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sucrose palatability did not vary across sessions .
	manualset3
149091	2	407700	13	NULL	NULL	NULL	NULL	sessions	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Sucrose palatability did not vary across sessions .
	manualset3
149092	1	407701	13	NULL	NULL	0	NULL	enlargement 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sudden enlargement of EAH lesions with or without pain has been noted during puberty and pregnancy and has been attributed to hormonal stimulation .
	manualset3
149093	2	407701	13	NULL	NULL	0	NULL	EAH lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sudden enlargement of EAH lesions with or without pain has been noted during puberty and pregnancy and has been attributed to hormonal stimulation .
	manualset3
149094	3	407701	13	NULL	NULL	0	NULL	pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sudden enlargement of EAH lesions with or without pain has been noted during puberty and pregnancy and has been attributed to hormonal stimulation .
	manualset3
149095	4	407701	13	NULL	NULL	0	NULL	puberty	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Sudden enlargement of EAH lesions with or without pain has been noted during puberty and pregnancy and has been attributed to hormonal stimulation .
	manualset3
149096	5	407701	13	NULL	NULL	0	NULL	pregnancy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sudden enlargement of EAH lesions with or without pain has been noted during puberty and pregnancy and has been attributed to hormonal stimulation .
	manualset3
149097	6	407701	13	NULL	NULL	0	NULL	hormonal stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sudden enlargement of EAH lesions with or without pain has been noted during puberty and pregnancy and has been attributed to hormonal stimulation .
	manualset3
149098	1	407702	13	NULL	NULL	0	NULL	contraction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sudden resistive contraction of the tibialis posterior muscle is considered to be the mechanical cause of the initial traumatic injury , and a shallow tibialis posterior tendon sulcus may be the predisposing factor .
	manualset3
149099	2	407702	13	NULL	NULL	0	NULL	tibialis posterior muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Sudden resistive contraction of the tibialis posterior muscle is considered to be the mechanical cause of the initial traumatic injury , and a shallow tibialis posterior tendon sulcus may be the predisposing factor .
	manualset3
149100	3	407702	13	NULL	NULL	0	NULL	cause	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sudden resistive contraction of the tibialis posterior muscle is considered to be the mechanical cause of the initial traumatic injury , and a shallow tibialis posterior tendon sulcus may be the predisposing factor .
	manualset3
149101	4	407702	13	NULL	NULL	0	NULL	traumatic injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sudden resistive contraction of the tibialis posterior muscle is considered to be the mechanical cause of the initial traumatic injury , and a shallow tibialis posterior tendon sulcus may be the predisposing factor .
	manualset3
149102	5	407702	13	NULL	NULL	0	NULL	shallow tibialis posterior tendon sulcus 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sudden resistive contraction of the tibialis posterior muscle is considered to be the mechanical cause of the initial traumatic injury , and a shallow tibialis posterior tendon sulcus may be the predisposing factor .
	manualset3
149103	6	407702	13	NULL	NULL	NULL	NULL	factor	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Sudden resistive contraction of the tibialis posterior muscle is considered to be the mechanical cause of the initial traumatic injury , and a shallow tibialis posterior tendon sulcus may be the predisposing factor .
	manualset3
149104	1	407703	13	NULL	NULL	0	NULL	Sudden unexpected death in epilepsy ( SUDEP )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sudden unexpected death in epilepsy ( SUDEP ) is the leading cause of mortality in patients with chronic uncontrolled epilepsy .
	manualset3
149105	2	407703	13	NULL	NULL	0	NULL	cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sudden unexpected death in epilepsy ( SUDEP ) is the leading cause of mortality in patients with chronic uncontrolled epilepsy .
	manualset3
149106	3	407703	13	NULL	NULL	0	NULL	mortality 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sudden unexpected death in epilepsy ( SUDEP ) is the leading cause of mortality in patients with chronic uncontrolled epilepsy .
	manualset3
149107	4	407703	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sudden unexpected death in epilepsy ( SUDEP ) is the leading cause of mortality in patients with chronic uncontrolled epilepsy .
	manualset3
149108	5	407703	13	NULL	NULL	0	NULL	chronic uncontrolled epilepsy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Sudden unexpected death in epilepsy ( SUDEP ) is the leading cause of mortality in patients with chronic uncontrolled epilepsy .
	manualset3
149109	1	407704	13	NULL	NULL	0	NULL	Sulfate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfate and thiosulfate supported growth with formate or hydrogen as the electron donor and thus are probably respiratory electron acceptors .
	manualset3
149110	2	407704	13	NULL	NULL	0	NULL	thiosulfate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfate and thiosulfate supported growth with formate or hydrogen as the electron donor and thus are probably respiratory electron acceptors .
	manualset3
149111	3	407704	13	NULL	NULL	0	NULL	growth	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfate and thiosulfate supported growth with formate or hydrogen as the electron donor and thus are probably respiratory electron acceptors .
	manualset3
149112	4	407704	13	NULL	NULL	0	NULL	formate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfate and thiosulfate supported growth with formate or hydrogen as the electron donor and thus are probably respiratory electron acceptors .
	manualset3
149113	5	407704	13	NULL	NULL	NULL	NULL	hydrogen	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Sulfate and thiosulfate supported growth with formate or hydrogen as the electron donor and thus are probably respiratory electron acceptors .
	manualset3
149114	6	407704	13	NULL	NULL	0	NULL	electron donor 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfate and thiosulfate supported growth with formate or hydrogen as the electron donor and thus are probably respiratory electron acceptors .
	manualset3
149115	7	407704	13	NULL	NULL	0	NULL	respiratory electron acceptors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfate and thiosulfate supported growth with formate or hydrogen as the electron donor and thus are probably respiratory electron acceptors .
	manualset3
149116	1	407705	13	NULL	NULL	0	NULL	Sulfhydryl-alkylating reagents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfhydryl-alkylating reagents are known to inactivate the NAD glycohydrolase and ADP-ribosyltransferase activities of the S1 subunit of pertussis toxin , a protein which contains two cysteines at positions 41 and 200 .
	manualset3
149117	2	407705	13	NULL	NULL	0	NULL	NAD glycohydrolase activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfhydryl-alkylating reagents are known to inactivate the NAD glycohydrolase and ADP-ribosyltransferase activities of the S1 subunit of pertussis toxin , a protein which contains two cysteines at positions 41 and 200 .
	manualset3
149118	3	407705	13	NULL	NULL	0	NULL	ADP-ribosyltransferase activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfhydryl-alkylating reagents are known to inactivate the NAD glycohydrolase and ADP-ribosyltransferase activities of the S1 subunit of pertussis toxin , a protein which contains two cysteines at positions 41 and 200 .
	manualset3
149119	4	407705	13	NULL	NULL	0	NULL	S1 subunit of pertussis toxin	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfhydryl-alkylating reagents are known to inactivate the NAD glycohydrolase and ADP-ribosyltransferase activities of the S1 subunit of pertussis toxin , a protein which contains two cysteines at positions 41 and 200 .
	manualset3
149120	5	407705	13	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfhydryl-alkylating reagents are known to inactivate the NAD glycohydrolase and ADP-ribosyltransferase activities of the S1 subunit of pertussis toxin , a protein which contains two cysteines at positions 41 and 200 .
	manualset3
149121	6	407705	13	NULL	NULL	0	NULL	two 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfhydryl-alkylating reagents are known to inactivate the NAD glycohydrolase and ADP-ribosyltransferase activities of the S1 subunit of pertussis toxin , a protein which contains two cysteines at positions 41 and 200 .
	manualset3
149122	7	407705	13	NULL	NULL	0	NULL	cysteines	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfhydryl-alkylating reagents are known to inactivate the NAD glycohydrolase and ADP-ribosyltransferase activities of the S1 subunit of pertussis toxin , a protein which contains two cysteines at positions 41 and 200 .
	manualset3
149123	8	407705	13	NULL	NULL	0	NULL	positions 41	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfhydryl-alkylating reagents are known to inactivate the NAD glycohydrolase and ADP-ribosyltransferase activities of the S1 subunit of pertussis toxin , a protein which contains two cysteines at positions 41 and 200 .
	manualset3
149124	9	407705	13	NULL	NULL	0	NULL	positions 200	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfhydryl-alkylating reagents are known to inactivate the NAD glycohydrolase and ADP-ribosyltransferase activities of the S1 subunit of pertussis toxin , a protein which contains two cysteines at positions 41 and 200 .
	manualset3
149125	1	407706	13	NULL	NULL	0	NULL	Changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Changes in oxidative processes in the brain under the effect of certain parameters of stable noise ) .
	manualset3
149126	2	407706	13	NULL	NULL	0	NULL	oxidative processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Changes in oxidative processes in the brain under the effect of certain parameters of stable noise ) .
	manualset3
149127	3	407706	13	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Changes in oxidative processes in the brain under the effect of certain parameters of stable noise ) .
	manualset3
149128	4	407706	13	NULL	NULL	0	NULL	effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Changes in oxidative processes in the brain under the effect of certain parameters of stable noise ) .
	manualset3
149129	5	407706	13	NULL	NULL	0	NULL	parameters	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( Changes in oxidative processes in the brain under the effect of certain parameters of stable noise ) .
	manualset3
149130	6	407706	13	NULL	NULL	0	NULL	noise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Changes in oxidative processes in the brain under the effect of certain parameters of stable noise ) .
	manualset3
149131	1	407707	13	NULL	NULL	0	NULL	predictor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A powerful and easy-to-use predictor of 30-day mortality .
	manualset3
149132	2	407707	13	NULL	NULL	0	NULL	30-day 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A powerful and easy-to-use predictor of 30-day mortality .
	manualset3
149133	3	407707	13	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A powerful and easy-to-use predictor of 30-day mortality .
	manualset3
149134	1	407708	13	NULL	NULL	0	NULL	Sulfonylureas	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfonylureas have been the most widely prescribed first-line treatment for type 2 diabetes , although there is increasing use of combination therapy and of insulin .
	manualset3
149135	2	407708	13	NULL	NULL	0	NULL	first-line treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfonylureas have been the most widely prescribed first-line treatment for type 2 diabetes , although there is increasing use of combination therapy and of insulin .
	manualset3
149136	3	407708	13	NULL	NULL	0	NULL	type 2 diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfonylureas have been the most widely prescribed first-line treatment for type 2 diabetes , although there is increasing use of combination therapy and of insulin .
	manualset3
149137	4	407708	13	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfonylureas have been the most widely prescribed first-line treatment for type 2 diabetes , although there is increasing use of combination therapy and of insulin .
	manualset3
149138	5	407708	13	NULL	NULL	0	NULL	combination therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfonylureas have been the most widely prescribed first-line treatment for type 2 diabetes , although there is increasing use of combination therapy and of insulin .
	manualset3
149139	6	407708	13	NULL	NULL	0	NULL	insulin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfonylureas have been the most widely prescribed first-line treatment for type 2 diabetes , although there is increasing use of combination therapy and of insulin .
	manualset3
149140	1	407709	13	NULL	NULL	0	NULL	Sulfur dioxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfur dioxide and asthma -- a double-edged sword ?
	manualset3
149141	2	407709	13	NULL	NULL	0	NULL	asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfur dioxide and asthma -- a double-edged sword ?
	manualset3
149142	3	407709	13	NULL	NULL	0	NULL	sword	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfur dioxide and asthma -- a double-edged sword ?
	manualset3
149143	1	407710	13	NULL	NULL	0	NULL	Sulfur	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfur reacts readily with cholesterol at 150 degrees C , and the product of the reaction contains aromatic hydrocarbons , some with a benzene , some a naphthalene , and some a phenanthrene ring system as part of the molecule .
	manualset3
149144	2	407710	13	NULL	NULL	0	NULL	cholesterol 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfur reacts readily with cholesterol at 150 degrees C , and the product of the reaction contains aromatic hydrocarbons , some with a benzene , some a naphthalene , and some a phenanthrene ring system as part of the molecule .
	manualset3
149145	3	407710	13	NULL	NULL	0	NULL	150 degrees C 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfur reacts readily with cholesterol at 150 degrees C , and the product of the reaction contains aromatic hydrocarbons , some with a benzene , some a naphthalene , and some a phenanthrene ring system as part of the molecule .
	manualset3
149146	4	407710	13	NULL	NULL	0	NULL	product 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfur reacts readily with cholesterol at 150 degrees C , and the product of the reaction contains aromatic hydrocarbons , some with a benzene , some a naphthalene , and some a phenanthrene ring system as part of the molecule .
	manualset3
149147	5	407710	13	NULL	NULL	0	NULL	reaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfur reacts readily with cholesterol at 150 degrees C , and the product of the reaction contains aromatic hydrocarbons , some with a benzene , some a naphthalene , and some a phenanthrene ring system as part of the molecule .
	manualset3
149148	6	407710	13	NULL	NULL	0	NULL	aromatic hydrocarbons	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfur reacts readily with cholesterol at 150 degrees C , and the product of the reaction contains aromatic hydrocarbons , some with a benzene , some a naphthalene , and some a phenanthrene ring system as part of the molecule .
	manualset3
149149	7	407710	13	NULL	NULL	0	NULL	benzene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfur reacts readily with cholesterol at 150 degrees C , and the product of the reaction contains aromatic hydrocarbons , some with a benzene , some a naphthalene , and some a phenanthrene ring system as part of the molecule .
	manualset3
149150	8	407710	13	NULL	NULL	0	NULL	naphthalene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfur reacts readily with cholesterol at 150 degrees C , and the product of the reaction contains aromatic hydrocarbons , some with a benzene , some a naphthalene , and some a phenanthrene ring system as part of the molecule .
	manualset3
149151	9	407710	13	NULL	NULL	0	NULL	phenanthrene ring system	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfur reacts readily with cholesterol at 150 degrees C , and the product of the reaction contains aromatic hydrocarbons , some with a benzene , some a naphthalene , and some a phenanthrene ring system as part of the molecule .
	manualset3
149152	10	407710	13	NULL	NULL	0	NULL	part of the molecule	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sulfur reacts readily with cholesterol at 150 degrees C , and the product of the reaction contains aromatic hydrocarbons , some with a benzene , some a naphthalene , and some a phenanthrene ring system as part of the molecule .
	manualset3
149153	1	407711	13	NULL	NULL	0	NULL	Summary	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Summary : We describe a carotid-cavernous fistula ( CCF ) in a middle aged woman with Ehlers-Danlos syndrome ( EDS ) type IV , which manifested with a left-sided ophthalmoplegia .
	manualset3
149155	3	407711	13	NULL	NULL	0	NULL	middle aged woman	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Summary : We describe a carotid-cavernous fistula ( CCF ) in a middle aged woman with Ehlers-Danlos syndrome ( EDS ) type IV , which manifested with a left-sided ophthalmoplegia .
	manualset3
149156	4	407711	13	NULL	NULL	0	NULL	Ehlers-Danlos syndrome ( EDS ) type IV	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Summary : We describe a carotid-cavernous fistula ( CCF ) in a middle aged woman with Ehlers-Danlos syndrome ( EDS ) type IV , which manifested with a left-sided ophthalmoplegia .
	manualset3
149157	5	407711	13	NULL	NULL	0	NULL	left-sided ophthalmoplegia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Summary : We describe a carotid-cavernous fistula ( CCF ) in a middle aged woman with Ehlers-Danlos syndrome ( EDS ) type IV , which manifested with a left-sided ophthalmoplegia .
	manualset3
151652	6	407711	13	NULL	NULL	0	NULL	carotid-cavernous fistula ( CCF ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Summary : We describe a carotid-cavernous fistula ( CCF ) in a middle aged woman with Ehlers-Danlos syndrome ( EDS ) type IV , which manifested with a left-sided ophthalmoplegia .
	manualset3
149154	1	407712	13	NULL	NULL	NULL	NULL	Summary 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Summary -- Ru-Vert , a combination product , containing in each tablet , 25 mg of pentylenetetrazol , 12.5 mg of pheniramine maleate , and 50 mg of nictonic acid , was evaluated in the treatment of seventeen patients with benign paroxysmal positional vertigo .
	manualset3
149158	2	407712	13	NULL	NULL	0	NULL	Ru-Vert	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Summary -- Ru-Vert , a combination product , containing in each tablet , 25 mg of pentylenetetrazol , 12.5 mg of pheniramine maleate , and 50 mg of nictonic acid , was evaluated in the treatment of seventeen patients with benign paroxysmal positional vertigo .
	manualset3
149159	3	407712	13	NULL	NULL	0	NULL	combination product	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Summary -- Ru-Vert , a combination product , containing in each tablet , 25 mg of pentylenetetrazol , 12.5 mg of pheniramine maleate , and 50 mg of nictonic acid , was evaluated in the treatment of seventeen patients with benign paroxysmal positional vertigo .
	manualset3
149160	4	407712	13	NULL	NULL	0	NULL	tablet	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Summary -- Ru-Vert , a combination product , containing in each tablet , 25 mg of pentylenetetrazol , 12.5 mg of pheniramine maleate , and 50 mg of nictonic acid , was evaluated in the treatment of seventeen patients with benign paroxysmal positional vertigo .
	manualset3
149161	5	407712	13	NULL	NULL	0	NULL	25 mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Summary -- Ru-Vert , a combination product , containing in each tablet , 25 mg of pentylenetetrazol , 12.5 mg of pheniramine maleate , and 50 mg of nictonic acid , was evaluated in the treatment of seventeen patients with benign paroxysmal positional vertigo .
	manualset3
149162	6	407712	13	NULL	NULL	0	NULL	pentylenetetrazol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Summary -- Ru-Vert , a combination product , containing in each tablet , 25 mg of pentylenetetrazol , 12.5 mg of pheniramine maleate , and 50 mg of nictonic acid , was evaluated in the treatment of seventeen patients with benign paroxysmal positional vertigo .
	manualset3
149163	7	407712	13	NULL	NULL	0	NULL	12.5 mg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Summary -- Ru-Vert , a combination product , containing in each tablet , 25 mg of pentylenetetrazol , 12.5 mg of pheniramine maleate , and 50 mg of nictonic acid , was evaluated in the treatment of seventeen patients with benign paroxysmal positional vertigo .
	manualset3
149164	8	407712	13	NULL	NULL	0	NULL	pheniramine maleate	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Summary -- Ru-Vert , a combination product , containing in each tablet , 25 mg of pentylenetetrazol , 12.5 mg of pheniramine maleate , and 50 mg of nictonic acid , was evaluated in the treatment of seventeen patients with benign paroxysmal positional vertigo .
	manualset3
149165	9	407712	13	NULL	NULL	0	NULL	50 mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Summary -- Ru-Vert , a combination product , containing in each tablet , 25 mg of pentylenetetrazol , 12.5 mg of pheniramine maleate , and 50 mg of nictonic acid , was evaluated in the treatment of seventeen patients with benign paroxysmal positional vertigo .
	manualset3
149166	10	407712	13	NULL	NULL	0	NULL	nictonic acid 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Summary -- Ru-Vert , a combination product , containing in each tablet , 25 mg of pentylenetetrazol , 12.5 mg of pheniramine maleate , and 50 mg of nictonic acid , was evaluated in the treatment of seventeen patients with benign paroxysmal positional vertigo .
	manualset3
149167	11	407712	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Summary -- Ru-Vert , a combination product , containing in each tablet , 25 mg of pentylenetetrazol , 12.5 mg of pheniramine maleate , and 50 mg of nictonic acid , was evaluated in the treatment of seventeen patients with benign paroxysmal positional vertigo .
	manualset3
149168	12	407712	13	NULL	NULL	0	NULL	seventeen patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Summary -- Ru-Vert , a combination product , containing in each tablet , 25 mg of pentylenetetrazol , 12.5 mg of pheniramine maleate , and 50 mg of nictonic acid , was evaluated in the treatment of seventeen patients with benign paroxysmal positional vertigo .
	manualset3
149169	13	407712	13	NULL	NULL	0	NULL	benign paroxysmal positional vertigo	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Summary -- Ru-Vert , a combination product , containing in each tablet , 25 mg of pentylenetetrazol , 12.5 mg of pheniramine maleate , and 50 mg of nictonic acid , was evaluated in the treatment of seventeen patients with benign paroxysmal positional vertigo .
	manualset3
149170	1	407713	13	NULL	NULL	0	NULL	Summation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Summation of XbaI fragments from five E. coli O157 : H7 strains estimated the genomic length at ca .
	manualset3
149171	2	407713	13	NULL	NULL	0	NULL	XbaI fragments	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Summation of XbaI fragments from five E. coli O157 : H7 strains estimated the genomic length at ca .
	manualset3
149172	3	407713	13	NULL	NULL	0	NULL	five	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Summation of XbaI fragments from five E. coli O157 : H7 strains estimated the genomic length at ca .
	manualset3
149173	4	407713	13	NULL	NULL	0	NULL	E. coli O157 : H7 strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Summation of XbaI fragments from five E. coli O157 : H7 strains estimated the genomic length at ca .
	manualset3
149174	5	407713	13	NULL	NULL	0	NULL	genomic length	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Summation of XbaI fragments from five E. coli O157 : H7 strains estimated the genomic length at ca .
	manualset3
149175	6	407713	13	NULL	NULL	0	NULL	ca	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Summation of XbaI fragments from five E. coli O157 : H7 strains estimated the genomic length at ca .
	manualset3
149176	1	407714	13	NULL	NULL	0	NULL	Summation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Summation of the signal intensity in each of the sections was carried out on the maps analogous to the analysis performed on V/Q scans and statistically compared using the Kendall 's tau rank correlation .
	manualset3
149177	2	407714	13	NULL	NULL	0	NULL	signal intensity 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Summation of the signal intensity in each of the sections was carried out on the maps analogous to the analysis performed on V/Q scans and statistically compared using the Kendall 's tau rank correlation .
	manualset3
149178	3	407714	13	NULL	NULL	0	NULL	sections	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Summation of the signal intensity in each of the sections was carried out on the maps analogous to the analysis performed on V/Q scans and statistically compared using the Kendall 's tau rank correlation .
	manualset3
149179	4	407714	13	NULL	NULL	0	NULL	maps	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Summation of the signal intensity in each of the sections was carried out on the maps analogous to the analysis performed on V/Q scans and statistically compared using the Kendall 's tau rank correlation .
	manualset3
149180	5	407714	13	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Summation of the signal intensity in each of the sections was carried out on the maps analogous to the analysis performed on V/Q scans and statistically compared using the Kendall 's tau rank correlation .
	manualset3
149181	6	407714	13	NULL	NULL	0	NULL	V/Q scans	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Summation of the signal intensity in each of the sections was carried out on the maps analogous to the analysis performed on V/Q scans and statistically compared using the Kendall 's tau rank correlation .
	manualset3
149182	7	407714	13	NULL	NULL	0	NULL	Kendall 's tau rank correlation	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Summation of the signal intensity in each of the sections was carried out on the maps analogous to the analysis performed on V/Q scans and statistically compared using the Kendall 's tau rank correlation .
	manualset3
149183	1	407715	13	NULL	NULL	NULL	NULL	light	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Superenhanced backscattering of light by nanoparticles .
	manualset3
149184	2	407715	13	NULL	NULL	0	NULL	nanoparticles 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Superenhanced backscattering of light by nanoparticles .
	manualset3
149185	1	407716	13	NULL	NULL	0	NULL	practice 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A practice ISWT is advocated but often omitted by PR centres .
	manualset3
149186	2	407716	13	NULL	NULL	0	NULL	ISWT	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A practice ISWT is advocated but often omitted by PR centres .
	manualset3
149187	3	407716	13	NULL	NULL	0	NULL	PR centres	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A practice ISWT is advocated but often omitted by PR centres .
	manualset3
149188	1	407717	13	NULL	NULL	NULL	NULL	Superfusion 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Superfusion of norepinephrine ( 1 nM - 10 microM ) hyperpolarized the cells in a concentration-dependent manner .
	manualset3
149189	2	407717	13	NULL	NULL	0	NULL	norepinephrine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Superfusion of norepinephrine ( 1 nM - 10 microM ) hyperpolarized the cells in a concentration-dependent manner .
	manualset3
149190	3	407717	13	NULL	NULL	0	NULL	1 nM - 10 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Superfusion of norepinephrine ( 1 nM - 10 microM ) hyperpolarized the cells in a concentration-dependent manner .
	manualset3
149191	4	407717	13	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Superfusion of norepinephrine ( 1 nM - 10 microM ) hyperpolarized the cells in a concentration-dependent manner .
	manualset3
149192	5	407717	13	NULL	NULL	0	NULL	manner	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Superfusion of norepinephrine ( 1 nM - 10 microM ) hyperpolarized the cells in a concentration-dependent manner .
	manualset3
149193	1	407718	13	NULL	NULL	0	NULL	Superior colliculi 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Superior colliculi involvement in poststroke unilateral spatial neglect : a pilot study .
	manualset3
149194	2	407718	13	NULL	NULL	0	NULL	involvement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Superior colliculi involvement in poststroke unilateral spatial neglect : a pilot study .
	manualset3
149195	3	407718	13	NULL	NULL	0	NULL	poststroke	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Superior colliculi involvement in poststroke unilateral spatial neglect : a pilot study .
	manualset3
149196	4	407718	13	NULL	NULL	0	NULL	 neglect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Superior colliculi involvement in poststroke unilateral spatial neglect : a pilot study .
	manualset3
149197	5	407718	13	NULL	NULL	0	NULL	pilot study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Superior colliculi involvement in poststroke unilateral spatial neglect : a pilot study .
	manualset3
149198	1	407719	13	NULL	NULL	0	NULL	Superior colliculus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Superior colliculus stimulation enhances neocortical serotonin release and electrocorticographic activation in the urethane-anesthetized rat .
	manualset3
149199	2	407719	13	NULL	NULL	0	NULL	stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Superior colliculus stimulation enhances neocortical serotonin release and electrocorticographic activation in the urethane-anesthetized rat .
	manualset3
149200	3	407719	13	NULL	NULL	0	NULL	neocortical serotonin release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Superior colliculus stimulation enhances neocortical serotonin release and electrocorticographic activation in the urethane-anesthetized rat .
	manualset3
149201	4	407719	13	NULL	NULL	0	NULL	electrocorticographic activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Superior colliculus stimulation enhances neocortical serotonin release and electrocorticographic activation in the urethane-anesthetized rat .
	manualset3
149202	5	407719	13	NULL	NULL	0	NULL	urethane-anesthetized rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Superior colliculus stimulation enhances neocortical serotonin release and electrocorticographic activation in the urethane-anesthetized rat .
	manualset3
149203	1	407720	13	NULL	NULL	0	NULL	Superior forniceal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Superior forniceal cells displayed higher colony-forming efficiency ( 3.6 % 0.9 % ) than superior bulbar ( 1.1 % 0.3 % ; P & lt ; 0.05 ) and inferior bulbar cells ( 1.6 % 0.8 % ; P & lt ; 0.05 ) .
	manualset3
149204	2	407720	13	NULL	NULL	0	NULL	efficiency	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Superior forniceal cells displayed higher colony-forming efficiency ( 3.6 % 0.9 % ) than superior bulbar ( 1.1 % 0.3 % ; P & lt ; 0.05 ) and inferior bulbar cells ( 1.6 % 0.8 % ; P & lt ; 0.05 ) .
	manualset3
149205	3	407720	13	NULL	NULL	0	NULL	3.6 % 0.9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Superior forniceal cells displayed higher colony-forming efficiency ( 3.6 % 0.9 % ) than superior bulbar ( 1.1 % 0.3 % ; P & lt ; 0.05 ) and inferior bulbar cells ( 1.6 % 0.8 % ; P & lt ; 0.05 ) .
	manualset3
149206	4	407720	13	NULL	NULL	0	NULL	superior bulbar	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Superior forniceal cells displayed higher colony-forming efficiency ( 3.6 % 0.9 % ) than superior bulbar ( 1.1 % 0.3 % ; P & lt ; 0.05 ) and inferior bulbar cells ( 1.6 % 0.8 % ; P & lt ; 0.05 ) .
	manualset3
149207	5	407720	13	NULL	NULL	0	NULL	1.1 % 0.3 % ; P & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Superior forniceal cells displayed higher colony-forming efficiency ( 3.6 % 0.9 % ) than superior bulbar ( 1.1 % 0.3 % ; P & lt ; 0.05 ) and inferior bulbar cells ( 1.6 % 0.8 % ; P & lt ; 0.05 ) .
	manualset3
149208	6	407720	13	NULL	NULL	0	NULL	inferior bulbar cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Superior forniceal cells displayed higher colony-forming efficiency ( 3.6 % 0.9 % ) than superior bulbar ( 1.1 % 0.3 % ; P & lt ; 0.05 ) and inferior bulbar cells ( 1.6 % 0.8 % ; P & lt ; 0.05 ) .
	manualset3
149209	7	407720	13	NULL	NULL	0	NULL	1.6 % 0.8 % ; P & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Superior forniceal cells displayed higher colony-forming efficiency ( 3.6 % 0.9 % ) than superior bulbar ( 1.1 % 0.3 % ; P & lt ; 0.05 ) and inferior bulbar cells ( 1.6 % 0.8 % ; P & lt ; 0.05 ) .
	manualset3
149277	1	407721	13	NULL	NULL	0	NULL	Supernatants	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Supernatants which inhibited the migration of peritoneal exudate macrophages had only minimal or no effect on the migration of alveolar macrophages , confirming that the inhibitory effects studied were attributable to MF and not cytophilic antibody .
	manualset3
149278	2	407721	13	NULL	NULL	0	NULL	migration 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Supernatants which inhibited the migration of peritoneal exudate macrophages had only minimal or no effect on the migration of alveolar macrophages , confirming that the inhibitory effects studied were attributable to MF and not cytophilic antibody .
	manualset3
149279	3	407721	13	NULL	NULL	0	NULL	peritoneal exudate macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Supernatants which inhibited the migration of peritoneal exudate macrophages had only minimal or no effect on the migration of alveolar macrophages , confirming that the inhibitory effects studied were attributable to MF and not cytophilic antibody .
	manualset3
149280	4	407721	13	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Supernatants which inhibited the migration of peritoneal exudate macrophages had only minimal or no effect on the migration of alveolar macrophages , confirming that the inhibitory effects studied were attributable to MF and not cytophilic antibody .
	manualset3
149281	5	407721	13	NULL	NULL	0	NULL	migration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Supernatants which inhibited the migration of peritoneal exudate macrophages had only minimal or no effect on the migration of alveolar macrophages , confirming that the inhibitory effects studied were attributable to MF and not cytophilic antibody .
	manualset3
149282	6	407721	13	NULL	NULL	0	NULL	alveolar macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Supernatants which inhibited the migration of peritoneal exudate macrophages had only minimal or no effect on the migration of alveolar macrophages , confirming that the inhibitory effects studied were attributable to MF and not cytophilic antibody .
	manualset3
149283	7	407721	13	NULL	NULL	0	NULL	 effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Supernatants which inhibited the migration of peritoneal exudate macrophages had only minimal or no effect on the migration of alveolar macrophages , confirming that the inhibitory effects studied were attributable to MF and not cytophilic antibody .
	manualset3
149284	8	407721	13	NULL	NULL	0	NULL	MF	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Supernatants which inhibited the migration of peritoneal exudate macrophages had only minimal or no effect on the migration of alveolar macrophages , confirming that the inhibitory effects studied were attributable to MF and not cytophilic antibody .
	manualset3
149285	9	407721	13	NULL	NULL	0	NULL	cytophilic antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Supernatants which inhibited the migration of peritoneal exudate macrophages had only minimal or no effect on the migration of alveolar macrophages , confirming that the inhibitory effects studied were attributable to MF and not cytophilic antibody .
	manualset3
149286	1	407722	13	NULL	NULL	0	NULL	Superovulated immature rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Superovulated immature rats ( 24 to 25 days old ) were inseminated with epididymal sperm before or after ovulation and their eggs were examined at various times .
	manualset3
149287	2	407722	13	NULL	NULL	0	NULL	24 to 25 days old	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Superovulated immature rats ( 24 to 25 days old ) were inseminated with epididymal sperm before or after ovulation and their eggs were examined at various times .
	manualset3
149288	3	407722	13	NULL	NULL	0	NULL	epididymal sperm	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Superovulated immature rats ( 24 to 25 days old ) were inseminated with epididymal sperm before or after ovulation and their eggs were examined at various times .
	manualset3
149289	4	407722	13	NULL	NULL	0	NULL	ovulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Superovulated immature rats ( 24 to 25 days old ) were inseminated with epididymal sperm before or after ovulation and their eggs were examined at various times .
	manualset3
149290	5	407722	13	NULL	NULL	0	NULL	eggs	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Superovulated immature rats ( 24 to 25 days old ) were inseminated with epididymal sperm before or after ovulation and their eggs were examined at various times .
	manualset3
149291	6	407722	13	NULL	NULL	0	NULL	various times 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Superovulated immature rats ( 24 to 25 days old ) were inseminated with epididymal sperm before or after ovulation and their eggs were examined at various times .
	manualset3
149292	1	407723	13	NULL	NULL	0	NULL	Superoxide anion	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Superoxide anion generation in Drosophila during melanotic encapsulation of parasites .
	manualset3
149293	2	407723	13	NULL	NULL	0	NULL	generation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Superoxide anion generation in Drosophila during melanotic encapsulation of parasites .
	manualset3
149294	3	407723	13	NULL	NULL	0	NULL	Drosophila	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Superoxide anion generation in Drosophila during melanotic encapsulation of parasites .
	manualset3
149295	4	407723	13	NULL	NULL	0	NULL	melanotic encapsulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Superoxide anion generation in Drosophila during melanotic encapsulation of parasites .
	manualset3
149296	5	407723	13	NULL	NULL	0	NULL	parasites	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Superoxide anion generation in Drosophila during melanotic encapsulation of parasites .
	manualset3
149297	1	407724	13	NULL	NULL	0	NULL	Superoxide	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Superoxide chemiluminescence and NF-kappaB activation were observed only at 2 wk post-MCT and both decreased by 4 wk post-MCT despite progressive PAH .
	manualset3
149298	2	407724	13	NULL	NULL	0	NULL	chemiluminescence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Superoxide chemiluminescence and NF-kappaB activation were observed only at 2 wk post-MCT and both decreased by 4 wk post-MCT despite progressive PAH .
	manualset3
149299	3	407724	13	NULL	NULL	0	NULL	NF-kappaB activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Superoxide chemiluminescence and NF-kappaB activation were observed only at 2 wk post-MCT and both decreased by 4 wk post-MCT despite progressive PAH .
	manualset3
149300	4	407724	13	NULL	NULL	0	NULL	2 wk post-MCT	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Superoxide chemiluminescence and NF-kappaB activation were observed only at 2 wk post-MCT and both decreased by 4 wk post-MCT despite progressive PAH .
	manualset3
149301	5	407724	13	NULL	NULL	0	NULL	4 wk post-MCT	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Superoxide chemiluminescence and NF-kappaB activation were observed only at 2 wk post-MCT and both decreased by 4 wk post-MCT despite progressive PAH .
	manualset3
149302	6	407724	13	NULL	NULL	0	NULL	progressive PAH	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Superoxide chemiluminescence and NF-kappaB activation were observed only at 2 wk post-MCT and both decreased by 4 wk post-MCT despite progressive PAH .
	manualset3
149303	1	407725	13	NULL	NULL	0	NULL	period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A preliminary period of intensive medical treatment before surgery may be advantageous since there is little evidence that survival rates are improved by treating unstable angina as an acute surgical emergency .
	manualset3
149304	2	407725	13	NULL	NULL	0	NULL	intensive medical treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A preliminary period of intensive medical treatment before surgery may be advantageous since there is little evidence that survival rates are improved by treating unstable angina as an acute surgical emergency .
	manualset3
149305	3	407725	13	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A preliminary period of intensive medical treatment before surgery may be advantageous since there is little evidence that survival rates are improved by treating unstable angina as an acute surgical emergency .
	manualset3
149306	4	407725	13	NULL	NULL	0	NULL	evidence 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A preliminary period of intensive medical treatment before surgery may be advantageous since there is little evidence that survival rates are improved by treating unstable angina as an acute surgical emergency .
	manualset3
149307	5	407725	13	NULL	NULL	0	NULL	survival rates	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A preliminary period of intensive medical treatment before surgery may be advantageous since there is little evidence that survival rates are improved by treating unstable angina as an acute surgical emergency .
	manualset3
149308	6	407725	13	NULL	NULL	0	NULL	unstable angina	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A preliminary period of intensive medical treatment before surgery may be advantageous since there is little evidence that survival rates are improved by treating unstable angina as an acute surgical emergency .
	manualset3
149309	7	407725	13	NULL	NULL	NULL	NULL	acute surgical emergency 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A preliminary period of intensive medical treatment before surgery may be advantageous since there is little evidence that survival rates are improved by treating unstable angina as an acute surgical emergency .
	manualset3
149310	1	407726	13	NULL	NULL	0	NULL	Superparamagnetic iron oxide ( SPIO )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Superparamagnetic iron oxide ( SPIO ) - enhanced MRI was performed in twenty-one patients undergoing proton-beam radiotherapy for hepatocellular carcinomas .
	manualset3
149311	2	407726	13	NULL	NULL	0	NULL	MRI	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Superparamagnetic iron oxide ( SPIO ) - enhanced MRI was performed in twenty-one patients undergoing proton-beam radiotherapy for hepatocellular carcinomas .
	manualset3
149312	3	407726	13	NULL	NULL	0	NULL	twenty-one 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Superparamagnetic iron oxide ( SPIO ) - enhanced MRI was performed in twenty-one patients undergoing proton-beam radiotherapy for hepatocellular carcinomas .
	manualset3
149313	4	407726	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Superparamagnetic iron oxide ( SPIO ) - enhanced MRI was performed in twenty-one patients undergoing proton-beam radiotherapy for hepatocellular carcinomas .
	manualset3
149314	5	407726	13	NULL	NULL	0	NULL	proton-beam radiotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Superparamagnetic iron oxide ( SPIO ) - enhanced MRI was performed in twenty-one patients undergoing proton-beam radiotherapy for hepatocellular carcinomas .
	manualset3
149315	6	407726	13	NULL	NULL	0	NULL	hepatocellular carcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Superparamagnetic iron oxide ( SPIO ) - enhanced MRI was performed in twenty-one patients undergoing proton-beam radiotherapy for hepatocellular carcinomas .
	manualset3
149316	1	407727	13	NULL	NULL	0	NULL	Supervisors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Supervisors of postgraduate students are increasingly likely to find themselves discussing whether or not the student should use a CAQDAS ( computer assisted qualitative data analysis system ) in their research .
	manualset3
149317	2	407727	13	NULL	NULL	0	NULL	postgraduate students	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Supervisors of postgraduate students are increasingly likely to find themselves discussing whether or not the student should use a CAQDAS ( computer assisted qualitative data analysis system ) in their research .
	manualset3
149318	3	407727	13	NULL	NULL	0	NULL	student 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Supervisors of postgraduate students are increasingly likely to find themselves discussing whether or not the student should use a CAQDAS ( computer assisted qualitative data analysis system ) in their research .
	manualset3
149319	4	407727	13	NULL	NULL	0	NULL	CAQDAS ( computer assisted qualitative data analysis system )	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Supervisors of postgraduate students are increasingly likely to find themselves discussing whether or not the student should use a CAQDAS ( computer assisted qualitative data analysis system ) in their research .
	manualset3
149320	5	407727	13	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Supervisors of postgraduate students are increasingly likely to find themselves discussing whether or not the student should use a CAQDAS ( computer assisted qualitative data analysis system ) in their research .
	manualset3
149321	1	407728	13	NULL	NULL	0	NULL	flora 3x	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Supplying the flora 3x resulted in more ` normal ' mice compared with mice which received the flora once or twice .
	manualset3
149322	2	407728	13	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Supplying the flora 3x resulted in more ` normal ' mice compared with mice which received the flora once or twice .
	manualset3
149323	3	407728	13	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Supplying the flora 3x resulted in more ` normal ' mice compared with mice which received the flora once or twice .
	manualset3
149324	4	407728	13	NULL	NULL	0	NULL	flora	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Supplying the flora 3x resulted in more ` normal ' mice compared with mice which received the flora once or twice .
	manualset3
149325	5	407728	13	NULL	NULL	0	NULL	once	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Supplying the flora 3x resulted in more ` normal ' mice compared with mice which received the flora once or twice .
	manualset3
149326	6	407728	13	NULL	NULL	0	NULL	twice	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Supplying the flora 3x resulted in more ` normal ' mice compared with mice which received the flora once or twice .
	manualset3
149327	1	407729	13	NULL	NULL	0	NULL	Support vector machines	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Support vector machines : development of QSAR models for predicting anti-HIV-1 activity of TIBO derivatives .
	manualset3
149328	2	407729	13	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Support vector machines : development of QSAR models for predicting anti-HIV-1 activity of TIBO derivatives .
	manualset3
149329	3	407729	13	NULL	NULL	0	NULL	QSAR models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Support vector machines : development of QSAR models for predicting anti-HIV-1 activity of TIBO derivatives .
	manualset3
149330	4	407729	13	NULL	NULL	0	NULL	anti-HIV-1 activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Support vector machines : development of QSAR models for predicting anti-HIV-1 activity of TIBO derivatives .
	manualset3
149331	5	407729	13	NULL	NULL	0	NULL	TIBO derivatives 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Support vector machines : development of QSAR models for predicting anti-HIV-1 activity of TIBO derivatives .
	manualset3
149332	1	407730	13	NULL	NULL	0	NULL	Support	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Support for this arrangement is provided from electron microscopy and from analysis of the pH-dissociation pattern .
	manualset3
149333	2	407730	13	NULL	NULL	0	NULL	arrangement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Support for this arrangement is provided from electron microscopy and from analysis of the pH-dissociation pattern .
	manualset3
149334	3	407730	13	NULL	NULL	0	NULL	electron microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Support for this arrangement is provided from electron microscopy and from analysis of the pH-dissociation pattern .
	manualset3
149335	4	407730	13	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Support for this arrangement is provided from electron microscopy and from analysis of the pH-dissociation pattern .
	manualset3
149336	5	407730	13	NULL	NULL	0	NULL	pH-dissociation pattern 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Support for this arrangement is provided from electron microscopy and from analysis of the pH-dissociation pattern .
	manualset3
151550	1	408031	13	NULL	NULL	0	NULL	Ten years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten years after its introduction , the technique of intra-focal pinning of fractures of the lower extremity of the radius is now widely used .
	manualset3
151551	2	408031	13	NULL	NULL	0	NULL	introduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten years after its introduction , the technique of intra-focal pinning of fractures of the lower extremity of the radius is now widely used .
	manualset3
151552	3	408031	13	NULL	NULL	0	NULL	technique of intra-focal pinning of fractures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten years after its introduction , the technique of intra-focal pinning of fractures of the lower extremity of the radius is now widely used .
	manualset3
151553	4	408031	13	NULL	NULL	0	NULL	 lower extremity of the radius	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten years after its introduction , the technique of intra-focal pinning of fractures of the lower extremity of the radius is now widely used .
	manualset3
151554	1	408032	13	NULL	NULL	0	NULL	Ten years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten years after the discovery of the hepatitis C virus ( HCV ) and its association with NANB hepatitis as a major cause of chronic liver disease worldwide , our knowledge of the natural history of hepatitis C is still limited .
	manualset3
151555	2	408032	13	NULL	NULL	0	NULL	discovery	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten years after the discovery of the hepatitis C virus ( HCV ) and its association with NANB hepatitis as a major cause of chronic liver disease worldwide , our knowledge of the natural history of hepatitis C is still limited .
	manualset3
151556	3	408032	13	NULL	NULL	0	NULL	hepatitis C virus ( HCV ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten years after the discovery of the hepatitis C virus ( HCV ) and its association with NANB hepatitis as a major cause of chronic liver disease worldwide , our knowledge of the natural history of hepatitis C is still limited .
	manualset3
151557	4	408032	13	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten years after the discovery of the hepatitis C virus ( HCV ) and its association with NANB hepatitis as a major cause of chronic liver disease worldwide , our knowledge of the natural history of hepatitis C is still limited .
	manualset3
151558	5	408032	13	NULL	NULL	NULL	NULL	NANB hepatitis 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ten years after the discovery of the hepatitis C virus ( HCV ) and its association with NANB hepatitis as a major cause of chronic liver disease worldwide , our knowledge of the natural history of hepatitis C is still limited .
	manualset3
151559	6	408032	13	NULL	NULL	0	NULL	cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten years after the discovery of the hepatitis C virus ( HCV ) and its association with NANB hepatitis as a major cause of chronic liver disease worldwide , our knowledge of the natural history of hepatitis C is still limited .
	manualset3
151560	7	408032	13	NULL	NULL	0	NULL	chronic liver disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten years after the discovery of the hepatitis C virus ( HCV ) and its association with NANB hepatitis as a major cause of chronic liver disease worldwide , our knowledge of the natural history of hepatitis C is still limited .
	manualset3
151561	8	408032	13	NULL	NULL	NULL	NULL	knowledge	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ten years after the discovery of the hepatitis C virus ( HCV ) and its association with NANB hepatitis as a major cause of chronic liver disease worldwide , our knowledge of the natural history of hepatitis C is still limited .
	manualset3
151562	9	408032	13	NULL	NULL	0	NULL	natural history	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten years after the discovery of the hepatitis C virus ( HCV ) and its association with NANB hepatitis as a major cause of chronic liver disease worldwide , our knowledge of the natural history of hepatitis C is still limited .
	manualset3
151563	10	408032	13	NULL	NULL	0	NULL	hepatitis C 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten years after the discovery of the hepatitis C virus ( HCV ) and its association with NANB hepatitis as a major cause of chronic liver disease worldwide , our knowledge of the natural history of hepatitis C is still limited .
	manualset3
151564	1	408033	13	NULL	NULL	0	NULL	Teneurin C-terminal associated peptides 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Teneurin C-terminal associated peptides : an enigmatic family of neuropeptides with structural similarity to the corticotropin-releasing factor and calcitonin families of peptides .
	manualset3
151565	2	408033	13	NULL	NULL	0	NULL	enigmatic family 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Teneurin C-terminal associated peptides : an enigmatic family of neuropeptides with structural similarity to the corticotropin-releasing factor and calcitonin families of peptides .
	manualset3
151566	3	408033	13	NULL	NULL	0	NULL	neuropeptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Teneurin C-terminal associated peptides : an enigmatic family of neuropeptides with structural similarity to the corticotropin-releasing factor and calcitonin families of peptides .
	manualset3
151567	4	408033	13	NULL	NULL	0	NULL	structural similarity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Teneurin C-terminal associated peptides : an enigmatic family of neuropeptides with structural similarity to the corticotropin-releasing factor and calcitonin families of peptides .
	manualset3
151568	5	408033	13	NULL	NULL	NULL	NULL	corticotropin-releasing factor	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Teneurin C-terminal associated peptides : an enigmatic family of neuropeptides with structural similarity to the corticotropin-releasing factor and calcitonin families of peptides .
	manualset3
151569	6	408033	13	NULL	NULL	0	NULL	calcitonin families of peptides 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Teneurin C-terminal associated peptides : an enigmatic family of neuropeptides with structural similarity to the corticotropin-releasing factor and calcitonin families of peptides .
	manualset3
151570	1	408034	13	NULL	NULL	0	NULL	Term pregnancy human placenta	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Term pregnancy human placenta contains hCG/LH receptor mRNA transcripts and immunoreactive receptor protein .
	manualset3
151571	2	408034	13	NULL	NULL	0	NULL	 hCG/LH receptor mRNA transcripts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Term pregnancy human placenta contains hCG/LH receptor mRNA transcripts and immunoreactive receptor protein .
	manualset3
151572	3	408034	13	NULL	NULL	0	NULL	immunoreactive receptor protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Term pregnancy human placenta contains hCG/LH receptor mRNA transcripts and immunoreactive receptor protein .
	manualset3
151573	1	408035	13	NULL	NULL	0	NULL	macrophage actin-associated tyrosine-phosphorylated protein ( MAYP ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Termed macrophage actin-associated tyrosine-phosphorylated protein ( MAYP ) , p37 is the major F-actin-associated protein that is tyrosine-phosphorylated in macrophages and is likely to play a role in regulating the CSF-1-induced reorganization of the actin cytoskeleton .
	manualset3
151574	2	408035	13	NULL	NULL	0	NULL	p37 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Termed macrophage actin-associated tyrosine-phosphorylated protein ( MAYP ) , p37 is the major F-actin-associated protein that is tyrosine-phosphorylated in macrophages and is likely to play a role in regulating the CSF-1-induced reorganization of the actin cytoskeleton .
	manualset3
151575	3	408035	13	NULL	NULL	0	NULL	major F-actin-associated protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Termed macrophage actin-associated tyrosine-phosphorylated protein ( MAYP ) , p37 is the major F-actin-associated protein that is tyrosine-phosphorylated in macrophages and is likely to play a role in regulating the CSF-1-induced reorganization of the actin cytoskeleton .
	manualset3
151576	4	408035	13	NULL	NULL	0	NULL	macrophages 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Termed macrophage actin-associated tyrosine-phosphorylated protein ( MAYP ) , p37 is the major F-actin-associated protein that is tyrosine-phosphorylated in macrophages and is likely to play a role in regulating the CSF-1-induced reorganization of the actin cytoskeleton .
	manualset3
151577	5	408035	13	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Termed macrophage actin-associated tyrosine-phosphorylated protein ( MAYP ) , p37 is the major F-actin-associated protein that is tyrosine-phosphorylated in macrophages and is likely to play a role in regulating the CSF-1-induced reorganization of the actin cytoskeleton .
	manualset3
151578	6	408035	13	NULL	NULL	0	NULL	CSF-1-induced reorganization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Termed macrophage actin-associated tyrosine-phosphorylated protein ( MAYP ) , p37 is the major F-actin-associated protein that is tyrosine-phosphorylated in macrophages and is likely to play a role in regulating the CSF-1-induced reorganization of the actin cytoskeleton .
	manualset3
151579	7	408035	13	NULL	NULL	0	NULL	actin cytoskeleton 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Termed macrophage actin-associated tyrosine-phosphorylated protein ( MAYP ) , p37 is the major F-actin-associated protein that is tyrosine-phosphorylated in macrophages and is likely to play a role in regulating the CSF-1-induced reorganization of the actin cytoskeleton .
	manualset3
151580	1	408036	13	NULL	NULL	0	NULL	Changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Changes of TNF-alpha and C ( 3 ) complements in patients with silicosis ) .
	manualset3
151581	2	408036	13	NULL	NULL	0	NULL	TNF-alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Changes of TNF-alpha and C ( 3 ) complements in patients with silicosis ) .
	manualset3
151582	3	408036	13	NULL	NULL	NULL	NULL	C ( 3 ) complements	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Changes of TNF-alpha and C ( 3 ) complements in patients with silicosis ) .
	manualset3
151583	4	408036	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Changes of TNF-alpha and C ( 3 ) complements in patients with silicosis ) .
	manualset3
151584	5	408036	13	NULL	NULL	0	NULL	silicosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Changes of TNF-alpha and C ( 3 ) complements in patients with silicosis ) .
	manualset3
151585	1	408037	13	NULL	NULL	0	NULL	quadratic line	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A quadratic line was fitted for QTc against time for each antimalarial therapy .
	manualset3
151586	2	408037	13	NULL	NULL	0	NULL	QTc 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A quadratic line was fitted for QTc against time for each antimalarial therapy .
	manualset3
151587	3	408037	13	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	A quadratic line was fitted for QTc against time for each antimalarial therapy .
	manualset3
151588	4	408037	13	NULL	NULL	0	NULL	antimalarial therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A quadratic line was fitted for QTc against time for each antimalarial therapy .
	manualset3
151589	1	408038	13	NULL	NULL	0	NULL	Terminal axon pathology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Terminal axon pathology in infantile neuroaxonal dystrophy .
	manualset3
151590	2	408038	13	NULL	NULL	0	NULL	 infantile neuroaxonal dystrophy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Terminal axon pathology in infantile neuroaxonal dystrophy .
	manualset3
151591	1	408039	13	NULL	NULL	0	NULL	Terminal sialic acid residues	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Terminal sialic acid residues on SIgA protect underlying carbohydrate residues from exposure and hydrolysis by exoglycosidases ( galactosidase and hexosaminidase ) .
	manualset3
151592	2	408039	13	NULL	NULL	0	NULL	SIgA 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Terminal sialic acid residues on SIgA protect underlying carbohydrate residues from exposure and hydrolysis by exoglycosidases ( galactosidase and hexosaminidase ) .
	manualset3
151593	3	408039	13	NULL	NULL	0	NULL	carbohydrate residues	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Terminal sialic acid residues on SIgA protect underlying carbohydrate residues from exposure and hydrolysis by exoglycosidases ( galactosidase and hexosaminidase ) .
	manualset3
151594	4	408039	13	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Terminal sialic acid residues on SIgA protect underlying carbohydrate residues from exposure and hydrolysis by exoglycosidases ( galactosidase and hexosaminidase ) .
	manualset3
151595	5	408039	13	NULL	NULL	0	NULL	hydrolysis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Terminal sialic acid residues on SIgA protect underlying carbohydrate residues from exposure and hydrolysis by exoglycosidases ( galactosidase and hexosaminidase ) .
	manualset3
151596	6	408039	13	NULL	NULL	0	NULL	exoglycosidases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Terminal sialic acid residues on SIgA protect underlying carbohydrate residues from exposure and hydrolysis by exoglycosidases ( galactosidase and hexosaminidase ) .
	manualset3
151597	7	408039	13	NULL	NULL	0	NULL	galactosidase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Terminal sialic acid residues on SIgA protect underlying carbohydrate residues from exposure and hydrolysis by exoglycosidases ( galactosidase and hexosaminidase ) .
	manualset3
151598	8	408039	13	NULL	NULL	0	NULL	hexosaminidase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Terminal sialic acid residues on SIgA protect underlying carbohydrate residues from exposure and hydrolysis by exoglycosidases ( galactosidase and hexosaminidase ) .
	manualset3
151599	1	408040	13	NULL	NULL	0	NULL	Test measurements	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Test measurements are made on a constantan wire and indium tin oxide ( ITO ) thin film for illustration .
	manualset3
151600	2	408040	13	NULL	NULL	0	NULL	constantan wire	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	Test measurements are made on a constantan wire and indium tin oxide ( ITO ) thin film for illustration .
	manualset3
151601	3	408040	13	NULL	NULL	0	NULL	indium tin oxide ( ITO ) thin film	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	Test measurements are made on a constantan wire and indium tin oxide ( ITO ) thin film for illustration .
	manualset3
151602	4	408040	13	NULL	NULL	0	NULL	illustration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Test measurements are made on a constantan wire and indium tin oxide ( ITO ) thin film for illustration .
	manualset3
151617	1	408041	13	NULL	NULL	0	NULL	Test results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Test results on simulated sedimentation-equilibrium data indicate that a 4-fold reduction in error may be typical over standard analyses techniques .
	manualset3
151618	2	408041	13	NULL	NULL	0	NULL	 simulated sedimentation-equilibrium data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Test results on simulated sedimentation-equilibrium data indicate that a 4-fold reduction in error may be typical over standard analyses techniques .
	manualset3
151619	3	408041	13	NULL	NULL	0	NULL	4-fold reduction	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Test results on simulated sedimentation-equilibrium data indicate that a 4-fold reduction in error may be typical over standard analyses techniques .
	manualset3
151620	4	408041	13	NULL	NULL	0	NULL	error	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Test results on simulated sedimentation-equilibrium data indicate that a 4-fold reduction in error may be typical over standard analyses techniques .
	manualset3
151621	5	408041	13	NULL	NULL	0	NULL	 standard analyses techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Test results on simulated sedimentation-equilibrium data indicate that a 4-fold reduction in error may be typical over standard analyses techniques .
	manualset3
151622	1	408042	13	NULL	NULL	0	NULL	Testicular histopathology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Testicular histopathology revealed atrophy of the testes with no spermatogenesis and absence of germ cells .
	manualset3
151623	2	408042	13	NULL	NULL	0	NULL	atrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Testicular histopathology revealed atrophy of the testes with no spermatogenesis and absence of germ cells .
	manualset3
151624	3	408042	13	NULL	NULL	0	NULL	testes 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Testicular histopathology revealed atrophy of the testes with no spermatogenesis and absence of germ cells .
	manualset3
151625	4	408042	13	NULL	NULL	0	NULL	spermatogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Testicular histopathology revealed atrophy of the testes with no spermatogenesis and absence of germ cells .
	manualset3
151626	5	408042	13	NULL	NULL	0	NULL	absence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Testicular histopathology revealed atrophy of the testes with no spermatogenesis and absence of germ cells .
	manualset3
151627	6	408042	13	NULL	NULL	0	NULL	germ cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Testicular histopathology revealed atrophy of the testes with no spermatogenesis and absence of germ cells .
	manualset3
151628	1	408043	13	NULL	NULL	0	NULL	Testicular innervation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Testicular innervation in the donkey is not uniform .
	manualset3
151629	2	408043	13	NULL	NULL	0	NULL	donkey	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Testicular innervation in the donkey is not uniform .
	manualset3
151630	1	408044	13	NULL	NULL	0	NULL	Testicular weight	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Testicular weight was modified by photoperiod and the size of the melatonin implant .
	manualset3
151631	2	408044	13	NULL	NULL	0	NULL	photoperiod	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Testicular weight was modified by photoperiod and the size of the melatonin implant .
	manualset3
151632	3	408044	13	NULL	NULL	0	NULL	size	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Testicular weight was modified by photoperiod and the size of the melatonin implant .
	manualset3
151633	4	408044	13	NULL	NULL	0	NULL	 melatonin implant 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Testicular weight was modified by photoperiod and the size of the melatonin implant .
	manualset3
151634	1	408045	13	NULL	NULL	0	NULL	theoretical model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Testing a theoretical model for examining the relationship between family adjustment and expatriates ' work adjustment .
	manualset3
151635	2	408045	13	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Testing a theoretical model for examining the relationship between family adjustment and expatriates ' work adjustment .
	manualset3
151636	3	408045	13	NULL	NULL	0	NULL	family adjustment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Testing a theoretical model for examining the relationship between family adjustment and expatriates ' work adjustment .
	manualset3
151637	4	408045	13	NULL	NULL	0	NULL	work adjustment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Testing a theoretical model for examining the relationship between family adjustment and expatriates ' work adjustment .
	manualset3
151638	1	408046	13	NULL	NULL	0	NULL	Testosterone-BSA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone-BSA triggered RhoA/B and Cdc42 activation in DU145 cells followed by stimulation of downstream effectors ROCK , LIMK2 and ADF/destrin .
	manualset3
151639	2	408046	13	NULL	NULL	0	NULL	RhoA/B	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone-BSA triggered RhoA/B and Cdc42 activation in DU145 cells followed by stimulation of downstream effectors ROCK , LIMK2 and ADF/destrin .
	manualset3
151640	3	408046	13	NULL	NULL	0	NULL	Cdc42	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone-BSA triggered RhoA/B and Cdc42 activation in DU145 cells followed by stimulation of downstream effectors ROCK , LIMK2 and ADF/destrin .
	manualset3
151641	4	408046	13	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone-BSA triggered RhoA/B and Cdc42 activation in DU145 cells followed by stimulation of downstream effectors ROCK , LIMK2 and ADF/destrin .
	manualset3
151642	5	408046	13	NULL	NULL	0	NULL	DU145 cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone-BSA triggered RhoA/B and Cdc42 activation in DU145 cells followed by stimulation of downstream effectors ROCK , LIMK2 and ADF/destrin .
	manualset3
151643	6	408046	13	NULL	NULL	0	NULL	stimulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone-BSA triggered RhoA/B and Cdc42 activation in DU145 cells followed by stimulation of downstream effectors ROCK , LIMK2 and ADF/destrin .
	manualset3
151644	7	408046	13	NULL	NULL	0	NULL	downstream effectors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone-BSA triggered RhoA/B and Cdc42 activation in DU145 cells followed by stimulation of downstream effectors ROCK , LIMK2 and ADF/destrin .
	manualset3
151645	8	408046	13	NULL	NULL	0	NULL	ROCK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone-BSA triggered RhoA/B and Cdc42 activation in DU145 cells followed by stimulation of downstream effectors ROCK , LIMK2 and ADF/destrin .
	manualset3
151646	9	408046	13	NULL	NULL	0	NULL	LIMK2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone-BSA triggered RhoA/B and Cdc42 activation in DU145 cells followed by stimulation of downstream effectors ROCK , LIMK2 and ADF/destrin .
	manualset3
151647	10	408046	13	NULL	NULL	0	NULL	ADF/destrin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone-BSA triggered RhoA/B and Cdc42 activation in DU145 cells followed by stimulation of downstream effectors ROCK , LIMK2 and ADF/destrin .
	manualset3
151648	1	408047	13	NULL	NULL	0	NULL	Testosterone 6beta-hydroxylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone 6beta-hydroxylation and tolbutamide methylhydroxylation activities were comparable in CHP and HUM liver microsomes .
	manualset3
151649	2	408047	13	NULL	NULL	0	NULL	tolbutamide methylhydroxylation activities 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone 6beta-hydroxylation and tolbutamide methylhydroxylation activities were comparable in CHP and HUM liver microsomes .
	manualset3
151653	3	408047	13	NULL	NULL	0	NULL	CHP	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone 6beta-hydroxylation and tolbutamide methylhydroxylation activities were comparable in CHP and HUM liver microsomes .
	manualset3
151654	4	408047	13	NULL	NULL	0	NULL	HUM	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone 6beta-hydroxylation and tolbutamide methylhydroxylation activities were comparable in CHP and HUM liver microsomes .
	manualset3
151655	5	408047	13	NULL	NULL	0	NULL	liver microsomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone 6beta-hydroxylation and tolbutamide methylhydroxylation activities were comparable in CHP and HUM liver microsomes .
	manualset3
151656	1	408048	13	NULL	NULL	0	NULL	Testosterone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone mediates satellite cell activation in denervated rat levator ani muscle .
	manualset3
151657	2	408048	13	NULL	NULL	0	NULL	satellite cell activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone mediates satellite cell activation in denervated rat levator ani muscle .
	manualset3
151658	3	408048	13	NULL	NULL	0	NULL	rat levator ani muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone mediates satellite cell activation in denervated rat levator ani muscle .
	manualset3
151659	1	408049	13	NULL	NULL	0	NULL	Testosterone metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone metabolism was investigated in fractions of human skin , enriched in epidermis , dermis , sebaceous glands , and sweat glands , by histologic sectioning of skin punch biopsies , and the results were compared with two culturable skin cells , i.e. , keratinocytes and fibroblasts .
	manualset3
151660	2	408049	13	NULL	NULL	0	NULL	fractions 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone metabolism was investigated in fractions of human skin , enriched in epidermis , dermis , sebaceous glands , and sweat glands , by histologic sectioning of skin punch biopsies , and the results were compared with two culturable skin cells , i.e. , keratinocytes and fibroblasts .
	manualset3
151661	3	408049	13	NULL	NULL	0	NULL	human skin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone metabolism was investigated in fractions of human skin , enriched in epidermis , dermis , sebaceous glands , and sweat glands , by histologic sectioning of skin punch biopsies , and the results were compared with two culturable skin cells , i.e. , keratinocytes and fibroblasts .
	manualset3
151662	4	408049	13	NULL	NULL	0	NULL	epidermis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone metabolism was investigated in fractions of human skin , enriched in epidermis , dermis , sebaceous glands , and sweat glands , by histologic sectioning of skin punch biopsies , and the results were compared with two culturable skin cells , i.e. , keratinocytes and fibroblasts .
	manualset3
151663	5	408049	13	NULL	NULL	0	NULL	dermis 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone metabolism was investigated in fractions of human skin , enriched in epidermis , dermis , sebaceous glands , and sweat glands , by histologic sectioning of skin punch biopsies , and the results were compared with two culturable skin cells , i.e. , keratinocytes and fibroblasts .
	manualset3
151664	6	408049	13	NULL	NULL	0	NULL	sebaceous glands 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone metabolism was investigated in fractions of human skin , enriched in epidermis , dermis , sebaceous glands , and sweat glands , by histologic sectioning of skin punch biopsies , and the results were compared with two culturable skin cells , i.e. , keratinocytes and fibroblasts .
	manualset3
151665	7	408049	13	NULL	NULL	0	NULL	sweat glands 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone metabolism was investigated in fractions of human skin , enriched in epidermis , dermis , sebaceous glands , and sweat glands , by histologic sectioning of skin punch biopsies , and the results were compared with two culturable skin cells , i.e. , keratinocytes and fibroblasts .
	manualset3
151666	8	408049	13	NULL	NULL	0	NULL	histologic sectioning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone metabolism was investigated in fractions of human skin , enriched in epidermis , dermis , sebaceous glands , and sweat glands , by histologic sectioning of skin punch biopsies , and the results were compared with two culturable skin cells , i.e. , keratinocytes and fibroblasts .
	manualset3
151667	9	408049	13	NULL	NULL	0	NULL	skin punch biopsies	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone metabolism was investigated in fractions of human skin , enriched in epidermis , dermis , sebaceous glands , and sweat glands , by histologic sectioning of skin punch biopsies , and the results were compared with two culturable skin cells , i.e. , keratinocytes and fibroblasts .
	manualset3
151668	10	408049	13	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone metabolism was investigated in fractions of human skin , enriched in epidermis , dermis , sebaceous glands , and sweat glands , by histologic sectioning of skin punch biopsies , and the results were compared with two culturable skin cells , i.e. , keratinocytes and fibroblasts .
	manualset3
151669	11	408049	13	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone metabolism was investigated in fractions of human skin , enriched in epidermis , dermis , sebaceous glands , and sweat glands , by histologic sectioning of skin punch biopsies , and the results were compared with two culturable skin cells , i.e. , keratinocytes and fibroblasts .
	manualset3
151670	12	408049	13	NULL	NULL	0	NULL	skin cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone metabolism was investigated in fractions of human skin , enriched in epidermis , dermis , sebaceous glands , and sweat glands , by histologic sectioning of skin punch biopsies , and the results were compared with two culturable skin cells , i.e. , keratinocytes and fibroblasts .
	manualset3
151671	13	408049	13	NULL	NULL	0	NULL	keratinocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone metabolism was investigated in fractions of human skin , enriched in epidermis , dermis , sebaceous glands , and sweat glands , by histologic sectioning of skin punch biopsies , and the results were compared with two culturable skin cells , i.e. , keratinocytes and fibroblasts .
	manualset3
151672	14	408049	13	NULL	NULL	0	NULL	fibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone metabolism was investigated in fractions of human skin , enriched in epidermis , dermis , sebaceous glands , and sweat glands , by histologic sectioning of skin punch biopsies , and the results were compared with two culturable skin cells , i.e. , keratinocytes and fibroblasts .
	manualset3
151673	1	408050	13	NULL	NULL	0	NULL	Testosterone treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone treatment per se produced about a 35 % reduction of HERG current compared with untreated oocytes .
	manualset3
151674	2	408050	13	NULL	NULL	0	NULL	35 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone treatment per se produced about a 35 % reduction of HERG current compared with untreated oocytes .
	manualset3
151675	3	408050	13	NULL	NULL	0	NULL	reduction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone treatment per se produced about a 35 % reduction of HERG current compared with untreated oocytes .
	manualset3
151676	4	408050	13	NULL	NULL	0	NULL	HERG 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone treatment per se produced about a 35 % reduction of HERG current compared with untreated oocytes .
	manualset3
151677	5	408050	13	NULL	NULL	0	NULL	oocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Testosterone treatment per se produced about a 35 % reduction of HERG current compared with untreated oocytes .
	manualset3
151678	1	408051	13	NULL	NULL	0	NULL	quantitative bioassay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A quantitative bioassay for nerve growth factor ( NGF ) activity employing a clonal pheochromocytoma cell line .
	manualset3
151679	2	408051	13	NULL	NULL	0	NULL	nerve growth factor ( NGF ) activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A quantitative bioassay for nerve growth factor ( NGF ) activity employing a clonal pheochromocytoma cell line .
	manualset3
151680	3	408051	13	NULL	NULL	0	NULL	clonal pheochromocytoma cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A quantitative bioassay for nerve growth factor ( NGF ) activity employing a clonal pheochromocytoma cell line .
	manualset3
151681	1	408052	13	NULL	NULL	0	NULL	Tests	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Tests in vitro showed that the antifibrinolytic agents epsilon-aminocaproic acid , Trasylol and soybean trypsin inhibitor act only as fast antiplasmins .
	manualset3
151682	2	408052	13	NULL	NULL	0	NULL	antifibrinolytic agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Tests in vitro showed that the antifibrinolytic agents epsilon-aminocaproic acid , Trasylol and soybean trypsin inhibitor act only as fast antiplasmins .
	manualset3
151683	3	408052	13	NULL	NULL	0	NULL	epsilon-aminocaproic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Tests in vitro showed that the antifibrinolytic agents epsilon-aminocaproic acid , Trasylol and soybean trypsin inhibitor act only as fast antiplasmins .
	manualset3
151684	4	408052	13	NULL	NULL	0	NULL	Trasylol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Tests in vitro showed that the antifibrinolytic agents epsilon-aminocaproic acid , Trasylol and soybean trypsin inhibitor act only as fast antiplasmins .
	manualset3
151685	5	408052	13	NULL	NULL	0	NULL	soybean trypsin inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Tests in vitro showed that the antifibrinolytic agents epsilon-aminocaproic acid , Trasylol and soybean trypsin inhibitor act only as fast antiplasmins .
	manualset3
151686	6	408052	13	NULL	NULL	0	NULL	antiplasmins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Tests in vitro showed that the antifibrinolytic agents epsilon-aminocaproic acid , Trasylol and soybean trypsin inhibitor act only as fast antiplasmins .
	manualset3
151687	1	408053	13	NULL	NULL	0	NULL	Tests	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Tests were carried out at different temperatures ( 24 , 45 , 60 , and 80 degrees C ) to determine if there was a synergistic effect of temperature and electric pulse treatment on the destruction of L. brevis .
	manualset3
151688	2	408053	13	NULL	NULL	0	NULL	temperatures	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Tests were carried out at different temperatures ( 24 , 45 , 60 , and 80 degrees C ) to determine if there was a synergistic effect of temperature and electric pulse treatment on the destruction of L. brevis .
	manualset3
151689	3	408053	13	NULL	NULL	0	NULL	24 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Tests were carried out at different temperatures ( 24 , 45 , 60 , and 80 degrees C ) to determine if there was a synergistic effect of temperature and electric pulse treatment on the destruction of L. brevis .
	manualset3
151690	4	408053	13	NULL	NULL	0	NULL	45 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Tests were carried out at different temperatures ( 24 , 45 , 60 , and 80 degrees C ) to determine if there was a synergistic effect of temperature and electric pulse treatment on the destruction of L. brevis .
	manualset3
151691	5	408053	13	NULL	NULL	0	NULL	60 degrees C 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Tests were carried out at different temperatures ( 24 , 45 , 60 , and 80 degrees C ) to determine if there was a synergistic effect of temperature and electric pulse treatment on the destruction of L. brevis .
	manualset3
151692	6	408053	13	NULL	NULL	0	NULL	80 degrees C 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Tests were carried out at different temperatures ( 24 , 45 , 60 , and 80 degrees C ) to determine if there was a synergistic effect of temperature and electric pulse treatment on the destruction of L. brevis .
	manualset3
151693	7	408053	13	NULL	NULL	0	NULL	synergistic effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Tests were carried out at different temperatures ( 24 , 45 , 60 , and 80 degrees C ) to determine if there was a synergistic effect of temperature and electric pulse treatment on the destruction of L. brevis .
	manualset3
151694	8	408053	13	NULL	NULL	0	NULL	temperature	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Tests were carried out at different temperatures ( 24 , 45 , 60 , and 80 degrees C ) to determine if there was a synergistic effect of temperature and electric pulse treatment on the destruction of L. brevis .
	manualset3
151695	9	408053	13	NULL	NULL	0	NULL	electric pulse treatment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Tests were carried out at different temperatures ( 24 , 45 , 60 , and 80 degrees C ) to determine if there was a synergistic effect of temperature and electric pulse treatment on the destruction of L. brevis .
	manualset3
151696	10	408053	13	NULL	NULL	0	NULL	destruction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Tests were carried out at different temperatures ( 24 , 45 , 60 , and 80 degrees C ) to determine if there was a synergistic effect of temperature and electric pulse treatment on the destruction of L. brevis .
	manualset3
151697	11	408053	13	NULL	NULL	0	NULL	L. brevis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Tests were carried out at different temperatures ( 24 , 45 , 60 , and 80 degrees C ) to determine if there was a synergistic effect of temperature and electric pulse treatment on the destruction of L. brevis .
	manualset3
151698	1	408054	13	NULL	NULL	0	NULL	Tetanic episodes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Tetanic episodes disappeared , but plasma levels of magnesium and potassium did not recover to normal range .
	manualset3
151699	2	408054	13	NULL	NULL	0	NULL	plasma levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Tetanic episodes disappeared , but plasma levels of magnesium and potassium did not recover to normal range .
	manualset3
151700	3	408054	13	NULL	NULL	0	NULL	magnesium 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Tetanic episodes disappeared , but plasma levels of magnesium and potassium did not recover to normal range .
	manualset3
151701	4	408054	13	NULL	NULL	0	NULL	potassium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Tetanic episodes disappeared , but plasma levels of magnesium and potassium did not recover to normal range .
	manualset3
151702	5	408054	13	NULL	NULL	0	NULL	normal range	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Tetanic episodes disappeared , but plasma levels of magnesium and potassium did not recover to normal range .
	manualset3
151703	1	408055	13	NULL	NULL	0	NULL	Tetrafluorosuccinate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Tetrafluorosuccinate and mercaptosuccinate inhibited urinary SF excretion and tissue fluorescence strongly .
	manualset3
151704	2	408055	13	NULL	NULL	0	NULL	mercaptosuccinate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Tetrafluorosuccinate and mercaptosuccinate inhibited urinary SF excretion and tissue fluorescence strongly .
	manualset3
151705	3	408055	13	NULL	NULL	0	NULL	urinary SF excretion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Tetrafluorosuccinate and mercaptosuccinate inhibited urinary SF excretion and tissue fluorescence strongly .
	manualset3
151706	4	408055	13	NULL	NULL	0	NULL	tissue fluorescence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Tetrafluorosuccinate and mercaptosuccinate inhibited urinary SF excretion and tissue fluorescence strongly .
	manualset3
151707	1	408056	13	NULL	NULL	0	NULL	Tetrazepam ( TZP )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Tetrazepam ( TZP ) suppressed rat and guinea-pig tracheal tone by 100 % and there was no difference in the relaxant effects against tone induced by 120 mM K + , carbachol ( 0.5 microM ) or histamine ( 100 microM ) .
	manualset3
151708	2	408056	13	NULL	NULL	0	NULL	rat tracheal tone	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Tetrazepam ( TZP ) suppressed rat and guinea-pig tracheal tone by 100 % and there was no difference in the relaxant effects against tone induced by 120 mM K + , carbachol ( 0.5 microM ) or histamine ( 100 microM ) .
	manualset3
151709	3	408056	13	NULL	NULL	0	NULL	guinea-pig tracheal tone	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Tetrazepam ( TZP ) suppressed rat and guinea-pig tracheal tone by 100 % and there was no difference in the relaxant effects against tone induced by 120 mM K + , carbachol ( 0.5 microM ) or histamine ( 100 microM ) .
	manualset3
151710	4	408056	13	NULL	NULL	0	NULL	100 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Tetrazepam ( TZP ) suppressed rat and guinea-pig tracheal tone by 100 % and there was no difference in the relaxant effects against tone induced by 120 mM K + , carbachol ( 0.5 microM ) or histamine ( 100 microM ) .
	manualset3
151711	5	408056	13	NULL	NULL	NULL	NULL	difference	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Tetrazepam ( TZP ) suppressed rat and guinea-pig tracheal tone by 100 % and there was no difference in the relaxant effects against tone induced by 120 mM K + , carbachol ( 0.5 microM ) or histamine ( 100 microM ) .
	manualset3
151712	6	408056	13	NULL	NULL	0	NULL	relaxant effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Tetrazepam ( TZP ) suppressed rat and guinea-pig tracheal tone by 100 % and there was no difference in the relaxant effects against tone induced by 120 mM K + , carbachol ( 0.5 microM ) or histamine ( 100 microM ) .
	manualset3
151713	7	408056	13	NULL	NULL	0	NULL	tone	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Tetrazepam ( TZP ) suppressed rat and guinea-pig tracheal tone by 100 % and there was no difference in the relaxant effects against tone induced by 120 mM K + , carbachol ( 0.5 microM ) or histamine ( 100 microM ) .
	manualset3
151714	8	408056	13	NULL	NULL	0	NULL	120 mM K + , carbachol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Tetrazepam ( TZP ) suppressed rat and guinea-pig tracheal tone by 100 % and there was no difference in the relaxant effects against tone induced by 120 mM K + , carbachol ( 0.5 microM ) or histamine ( 100 microM ) .
	manualset3
151715	9	408056	13	NULL	NULL	0	NULL	0.5 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Tetrazepam ( TZP ) suppressed rat and guinea-pig tracheal tone by 100 % and there was no difference in the relaxant effects against tone induced by 120 mM K + , carbachol ( 0.5 microM ) or histamine ( 100 microM ) .
	manualset3
151716	10	408056	13	NULL	NULL	0	NULL	histamine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Tetrazepam ( TZP ) suppressed rat and guinea-pig tracheal tone by 100 % and there was no difference in the relaxant effects against tone induced by 120 mM K + , carbachol ( 0.5 microM ) or histamine ( 100 microM ) .
	manualset3
151717	11	408056	13	NULL	NULL	0	NULL	100 microM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Tetrazepam ( TZP ) suppressed rat and guinea-pig tracheal tone by 100 % and there was no difference in the relaxant effects against tone induced by 120 mM K + , carbachol ( 0.5 microM ) or histamine ( 100 microM ) .
	manualset3
151718	1	408057	13	NULL	NULL	0	NULL	Textile sensors	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	Textile sensors , when embedded into clothing , can provide new ways of monitoring physiological signals , and improve the usability and comfort of such monitoring systems in the areas of medical , occupational health and sports .
	manualset3
151719	2	408057	13	NULL	NULL	0	NULL	clothing	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	Textile sensors , when embedded into clothing , can provide new ways of monitoring physiological signals , and improve the usability and comfort of such monitoring systems in the areas of medical , occupational health and sports .
	manualset3
151720	3	408057	13	NULL	NULL	0	NULL	new ways 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Textile sensors , when embedded into clothing , can provide new ways of monitoring physiological signals , and improve the usability and comfort of such monitoring systems in the areas of medical , occupational health and sports .
	manualset3
151721	4	408057	13	NULL	NULL	0	NULL	monitoring 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Textile sensors , when embedded into clothing , can provide new ways of monitoring physiological signals , and improve the usability and comfort of such monitoring systems in the areas of medical , occupational health and sports .
	manualset3
151723	5	408057	13	NULL	NULL	0	NULL	physiological signals	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Textile sensors , when embedded into clothing , can provide new ways of monitoring physiological signals , and improve the usability and comfort of such monitoring systems in the areas of medical , occupational health and sports .
	manualset3
151724	6	408057	13	NULL	NULL	0	NULL	usability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Textile sensors , when embedded into clothing , can provide new ways of monitoring physiological signals , and improve the usability and comfort of such monitoring systems in the areas of medical , occupational health and sports .
	manualset3
151725	7	408057	13	NULL	NULL	0	NULL	comfort 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Textile sensors , when embedded into clothing , can provide new ways of monitoring physiological signals , and improve the usability and comfort of such monitoring systems in the areas of medical , occupational health and sports .
	manualset3
151726	8	408057	13	NULL	NULL	0	NULL	monitoring systems	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Textile sensors , when embedded into clothing , can provide new ways of monitoring physiological signals , and improve the usability and comfort of such monitoring systems in the areas of medical , occupational health and sports .
	manualset3
151728	9	408057	13	NULL	NULL	0	NULL	areas	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Textile sensors , when embedded into clothing , can provide new ways of monitoring physiological signals , and improve the usability and comfort of such monitoring systems in the areas of medical , occupational health and sports .
	manualset3
151729	10	408057	13	NULL	NULL	0	NULL	medical	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Textile sensors , when embedded into clothing , can provide new ways of monitoring physiological signals , and improve the usability and comfort of such monitoring systems in the areas of medical , occupational health and sports .
	manualset3
151730	11	408057	13	NULL	NULL	0	NULL	occupational health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Textile sensors , when embedded into clothing , can provide new ways of monitoring physiological signals , and improve the usability and comfort of such monitoring systems in the areas of medical , occupational health and sports .
	manualset3
151731	12	408057	13	NULL	NULL	0	NULL	sports	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Textile sensors , when embedded into clothing , can provide new ways of monitoring physiological signals , and improve the usability and comfort of such monitoring systems in the areas of medical , occupational health and sports .
	manualset3
151747	1	408058	13	NULL	NULL	0	NULL	Th2 cytokine protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Th2 cytokine protein production by T cells showed no apparent change .
	manualset3
151748	2	408058	13	NULL	NULL	0	NULL	production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Th2 cytokine protein production by T cells showed no apparent change .
	manualset3
151749	3	408058	13	NULL	NULL	0	NULL	T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Th2 cytokine protein production by T cells showed no apparent change .
	manualset3
151750	4	408058	13	NULL	NULL	0	NULL	change 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Th2 cytokine protein production by T cells showed no apparent change .
	manualset3
151751	1	408059	13	NULL	NULL	0	NULL	Thalamocortical ( TC ) projections 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Thalamocortical ( TC ) projections provide the major pathway for ascending sensory information to the mammalian neocortex .
	manualset3
151752	2	408059	13	NULL	NULL	0	NULL	 major pathway	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thalamocortical ( TC ) projections provide the major pathway for ascending sensory information to the mammalian neocortex .
	manualset3
151753	3	408059	13	NULL	NULL	0	NULL	sensory information	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thalamocortical ( TC ) projections provide the major pathway for ascending sensory information to the mammalian neocortex .
	manualset3
151754	4	408059	13	NULL	NULL	0	NULL	mammalian neocortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Thalamocortical ( TC ) projections provide the major pathway for ascending sensory information to the mammalian neocortex .
	manualset3
151755	1	408060	13	NULL	NULL	0	NULL	quantitative measure	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A quantitative measure of the degree to which a particular metal drives metalloregulation of transcription is the allosteric coupling-free energy , G ( c ) .
	manualset3
151757	2	408060	13	NULL	NULL	0	NULL	degree	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A quantitative measure of the degree to which a particular metal drives metalloregulation of transcription is the allosteric coupling-free energy , G ( c ) .
	manualset3
151758	3	408060	13	NULL	NULL	0	NULL	metal 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	A quantitative measure of the degree to which a particular metal drives metalloregulation of transcription is the allosteric coupling-free energy , G ( c ) .
	manualset3
151759	4	408060	13	NULL	NULL	0	NULL	metalloregulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A quantitative measure of the degree to which a particular metal drives metalloregulation of transcription is the allosteric coupling-free energy , G ( c ) .
	manualset3
151760	5	408060	13	NULL	NULL	0	NULL	transcription 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A quantitative measure of the degree to which a particular metal drives metalloregulation of transcription is the allosteric coupling-free energy , G ( c ) .
	manualset3
151761	6	408060	13	NULL	NULL	0	NULL	allosteric coupling-free energy , G ( c )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A quantitative measure of the degree to which a particular metal drives metalloregulation of transcription is the allosteric coupling-free energy , G ( c ) .
	manualset3
151762	1	408061	13	NULL	NULL	0	NULL	Thalidomide 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Thalidomide and its analogs seem to be promising drugs for further treatment of biliary cirrhosis .
	manualset3
151763	2	408061	13	NULL	NULL	0	NULL	analogs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Thalidomide and its analogs seem to be promising drugs for further treatment of biliary cirrhosis .
	manualset3
151764	3	408061	13	NULL	NULL	0	NULL	drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Thalidomide and its analogs seem to be promising drugs for further treatment of biliary cirrhosis .
	manualset3
151765	4	408061	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Thalidomide and its analogs seem to be promising drugs for further treatment of biliary cirrhosis .
	manualset3
151766	5	408061	13	NULL	NULL	0	NULL	biliary cirrhosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Thalidomide and its analogs seem to be promising drugs for further treatment of biliary cirrhosis .
	manualset3
151768	1	408062	13	NULL	NULL	0	NULL	Thalidomide maintenance therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Thalidomide maintenance therapy after autologous stem cell transplantation improved the quality of response and increased progression-free survival ( PFS ) significantly in all 6 studies and overall survival ( OS ) in 3 of them .
	manualset3
151769	2	408062	13	NULL	NULL	0	NULL	autologous stem cell transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Thalidomide maintenance therapy after autologous stem cell transplantation improved the quality of response and increased progression-free survival ( PFS ) significantly in all 6 studies and overall survival ( OS ) in 3 of them .
	manualset3
151774	3	408062	13	NULL	NULL	0	NULL	quality of response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thalidomide maintenance therapy after autologous stem cell transplantation improved the quality of response and increased progression-free survival ( PFS ) significantly in all 6 studies and overall survival ( OS ) in 3 of them .
	manualset3
151775	4	408062	13	NULL	NULL	0	NULL	progression-free survival 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thalidomide maintenance therapy after autologous stem cell transplantation improved the quality of response and increased progression-free survival ( PFS ) significantly in all 6 studies and overall survival ( OS ) in 3 of them .
	manualset3
151776	5	408062	13	NULL	NULL	0	NULL	PFS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thalidomide maintenance therapy after autologous stem cell transplantation improved the quality of response and increased progression-free survival ( PFS ) significantly in all 6 studies and overall survival ( OS ) in 3 of them .
	manualset3
151778	6	408062	13	NULL	NULL	0	NULL	6 studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thalidomide maintenance therapy after autologous stem cell transplantation improved the quality of response and increased progression-free survival ( PFS ) significantly in all 6 studies and overall survival ( OS ) in 3 of them .
	manualset3
151779	7	408062	13	NULL	NULL	0	NULL	overall survival ( OS )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thalidomide maintenance therapy after autologous stem cell transplantation improved the quality of response and increased progression-free survival ( PFS ) significantly in all 6 studies and overall survival ( OS ) in 3 of them .
	manualset3
151780	8	408062	13	NULL	NULL	0	NULL	3 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thalidomide maintenance therapy after autologous stem cell transplantation improved the quality of response and increased progression-free survival ( PFS ) significantly in all 6 studies and overall survival ( OS ) in 3 of them .
	manualset3
151800	1	408063	13	NULL	NULL	0	NULL	Sl/Sld	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	That Sl/Sld and W/Wv mBMMC contain high steady-state levels of five granule protease transcripts expressed by the mature serosal , ear , and skin mast cells of their normal + / + littermates suggests that c-kit-mediated signal transduction is not essential for inducing transcription of these protease genes .
	manualset3
151801	2	408063	13	NULL	NULL	0	NULL	W/Wv mBMMC	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	That Sl/Sld and W/Wv mBMMC contain high steady-state levels of five granule protease transcripts expressed by the mature serosal , ear , and skin mast cells of their normal + / + littermates suggests that c-kit-mediated signal transduction is not essential for inducing transcription of these protease genes .
	manualset3
151802	3	408063	13	NULL	NULL	0	NULL	steady-state levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	That Sl/Sld and W/Wv mBMMC contain high steady-state levels of five granule protease transcripts expressed by the mature serosal , ear , and skin mast cells of their normal + / + littermates suggests that c-kit-mediated signal transduction is not essential for inducing transcription of these protease genes .
	manualset3
151803	4	408063	13	NULL	NULL	0	NULL	five	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	That Sl/Sld and W/Wv mBMMC contain high steady-state levels of five granule protease transcripts expressed by the mature serosal , ear , and skin mast cells of their normal + / + littermates suggests that c-kit-mediated signal transduction is not essential for inducing transcription of these protease genes .
	manualset3
151804	5	408063	13	NULL	NULL	0	NULL	granule protease transcripts 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	That Sl/Sld and W/Wv mBMMC contain high steady-state levels of five granule protease transcripts expressed by the mature serosal , ear , and skin mast cells of their normal + / + littermates suggests that c-kit-mediated signal transduction is not essential for inducing transcription of these protease genes .
	manualset3
151805	6	408063	13	NULL	NULL	0	NULL	mature serosal mast cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	That Sl/Sld and W/Wv mBMMC contain high steady-state levels of five granule protease transcripts expressed by the mature serosal , ear , and skin mast cells of their normal + / + littermates suggests that c-kit-mediated signal transduction is not essential for inducing transcription of these protease genes .
	manualset3
151806	7	408063	13	NULL	NULL	0	NULL	ear mast cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	That Sl/Sld and W/Wv mBMMC contain high steady-state levels of five granule protease transcripts expressed by the mature serosal , ear , and skin mast cells of their normal + / + littermates suggests that c-kit-mediated signal transduction is not essential for inducing transcription of these protease genes .
	manualset3
151807	8	408063	13	NULL	NULL	0	NULL	skin mast cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	That Sl/Sld and W/Wv mBMMC contain high steady-state levels of five granule protease transcripts expressed by the mature serosal , ear , and skin mast cells of their normal + / + littermates suggests that c-kit-mediated signal transduction is not essential for inducing transcription of these protease genes .
	manualset3
151808	9	408063	13	NULL	NULL	0	NULL	normal + / + littermates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	That Sl/Sld and W/Wv mBMMC contain high steady-state levels of five granule protease transcripts expressed by the mature serosal , ear , and skin mast cells of their normal + / + littermates suggests that c-kit-mediated signal transduction is not essential for inducing transcription of these protease genes .
	manualset3
151809	10	408063	13	NULL	NULL	0	NULL	c-kit-mediated signal transduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	That Sl/Sld and W/Wv mBMMC contain high steady-state levels of five granule protease transcripts expressed by the mature serosal , ear , and skin mast cells of their normal + / + littermates suggests that c-kit-mediated signal transduction is not essential for inducing transcription of these protease genes .
	manualset3
151810	11	408063	13	NULL	NULL	0	NULL	transcription 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	That Sl/Sld and W/Wv mBMMC contain high steady-state levels of five granule protease transcripts expressed by the mature serosal , ear , and skin mast cells of their normal + / + littermates suggests that c-kit-mediated signal transduction is not essential for inducing transcription of these protease genes .
	manualset3
151811	12	408063	13	NULL	NULL	0	NULL	protease genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	That Sl/Sld and W/Wv mBMMC contain high steady-state levels of five granule protease transcripts expressed by the mature serosal , ear , and skin mast cells of their normal + / + littermates suggests that c-kit-mediated signal transduction is not essential for inducing transcription of these protease genes .
	manualset3
151812	1	408064	13	NULL	NULL	0	NULL	physical link	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	That physical link between n and D throw a light on the nature of ultra-structure alterations occuring in the edematous stroma .
	manualset3
151813	2	408064	13	NULL	NULL	0	NULL	n 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	That physical link between n and D throw a light on the nature of ultra-structure alterations occuring in the edematous stroma .
	manualset3
151814	3	408064	13	NULL	NULL	0	NULL	D	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	That physical link between n and D throw a light on the nature of ultra-structure alterations occuring in the edematous stroma .
	manualset3
151815	4	408064	13	NULL	NULL	0	NULL	throw 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	That physical link between n and D throw a light on the nature of ultra-structure alterations occuring in the edematous stroma .
	manualset3
151816	5	408064	13	NULL	NULL	0	NULL	light	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	That physical link between n and D throw a light on the nature of ultra-structure alterations occuring in the edematous stroma .
	manualset3
151817	6	408064	13	NULL	NULL	0	NULL	nature	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	That physical link between n and D throw a light on the nature of ultra-structure alterations occuring in the edematous stroma .
	manualset3
151818	7	408064	13	NULL	NULL	0	NULL	ultra-structure alterations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	That physical link between n and D throw a light on the nature of ultra-structure alterations occuring in the edematous stroma .
	manualset3
151819	8	408064	13	NULL	NULL	0	NULL	edematous stroma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	That physical link between n and D throw a light on the nature of ultra-structure alterations occuring in the edematous stroma .
	manualset3
151820	1	408065	13	NULL	NULL	0	NULL	generation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	That is , the generation of CTL and TsN are inhibited while the induction of TsS is not .
	manualset3
151821	2	408065	13	NULL	NULL	0	NULL	CTL	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	That is , the generation of CTL and TsN are inhibited while the induction of TsS is not .
	manualset3
151822	3	408065	13	NULL	NULL	0	NULL	 TsN 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	That is , the generation of CTL and TsN are inhibited while the induction of TsS is not .
	manualset3
151823	4	408065	13	NULL	NULL	0	NULL	 induction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	That is , the generation of CTL and TsN are inhibited while the induction of TsS is not .
	manualset3
151824	5	408065	13	NULL	NULL	0	NULL	TsS 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	That is , the generation of CTL and TsN are inhibited while the induction of TsS is not .
	manualset3
151842	1	408066	13	NULL	NULL	0	NULL	neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	That is , these neurons responded to a tonal stimulus only if the stimulus was within a restricted range of both frequency and intensity .
	manualset3
151843	2	408066	13	NULL	NULL	0	NULL	tonal stimulus 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	That is , these neurons responded to a tonal stimulus only if the stimulus was within a restricted range of both frequency and intensity .
	manualset3
151844	3	408066	13	NULL	NULL	0	NULL	stimulus 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	That is , these neurons responded to a tonal stimulus only if the stimulus was within a restricted range of both frequency and intensity .
	manualset3
151845	4	408066	13	NULL	NULL	0	NULL	range	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	That is , these neurons responded to a tonal stimulus only if the stimulus was within a restricted range of both frequency and intensity .
	manualset3
151846	5	408066	13	NULL	NULL	0	NULL	frequency 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	That is , these neurons responded to a tonal stimulus only if the stimulus was within a restricted range of both frequency and intensity .
	manualset3
151847	6	408066	13	NULL	NULL	0	NULL	intensity 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	That is , these neurons responded to a tonal stimulus only if the stimulus was within a restricted range of both frequency and intensity .
	manualset3
151848	1	408067	13	NULL	NULL	0	NULL	quantitative model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A quantitative model based on a pulse-step controller , similar to that postulated for saccadic eye movements , has been developed to represent the initial component .
	manualset3
151849	2	408067	13	NULL	NULL	0	NULL	 pulse-step controller 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A quantitative model based on a pulse-step controller , similar to that postulated for saccadic eye movements , has been developed to represent the initial component .
	manualset3
151850	3	408067	13	NULL	NULL	0	NULL	 saccadic eye movements	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A quantitative model based on a pulse-step controller , similar to that postulated for saccadic eye movements , has been developed to represent the initial component .
	manualset3
151851	4	408067	13	NULL	NULL	0	NULL	initial component	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A quantitative model based on a pulse-step controller , similar to that postulated for saccadic eye movements , has been developed to represent the initial component .
	manualset3
151852	1	408068	13	NULL	NULL	0	NULL	mechanism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	That is why the actual causal mechanism of torture interrogation in curtailing terrorism must be elucidated by utilitarians rather than presumed
	manualset3
151853	2	408068	13	NULL	NULL	0	NULL	torture interrogation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	That is why the actual causal mechanism of torture interrogation in curtailing terrorism must be elucidated by utilitarians rather than presumed
	manualset3
151854	3	408068	13	NULL	NULL	0	NULL	terrorism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	That is why the actual causal mechanism of torture interrogation in curtailing terrorism must be elucidated by utilitarians rather than presumed
	manualset3
151855	4	408068	13	NULL	NULL	0	NULL	utilitarians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	That is why the actual causal mechanism of torture interrogation in curtailing terrorism must be elucidated by utilitarians rather than presumed
	manualset3
151856	1	408069	13	NULL	NULL	0	NULL	110	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	That means that there are still 110 WHO member states not using vaccine against HBV .
	manualset3
151857	2	408069	13	NULL	NULL	0	NULL	WHO member states	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	That means that there are still 110 WHO member states not using vaccine against HBV .
	manualset3
151858	3	408069	13	NULL	NULL	NULL	NULL	vaccine	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	That means that there are still 110 WHO member states not using vaccine against HBV .
	manualset3
151859	4	408069	13	NULL	NULL	0	NULL	HBV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	That means that there are still 110 WHO member states not using vaccine against HBV .
	manualset3
151860	1	408070	13	NULL	NULL	0	NULL	carboxyl terminal phenyl group	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	That the carboxyl terminal phenyl group was essential for reduction was shown by comparing variously substituted di - and tripeptides .
	manualset3
151861	2	408070	13	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	That the carboxyl terminal phenyl group was essential for reduction was shown by comparing variously substituted di - and tripeptides .
	manualset3
151862	3	408070	13	NULL	NULL	0	NULL	dipeptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	That the carboxyl terminal phenyl group was essential for reduction was shown by comparing variously substituted di - and tripeptides .
	manualset3
151863	4	408070	13	NULL	NULL	0	NULL	tripeptides 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	That the carboxyl terminal phenyl group was essential for reduction was shown by comparing variously substituted di - and tripeptides .
	manualset3
151864	1	408071	13	NULL	NULL	0	NULL	infected cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	That the infected cell at 44 C retained the capacity for synthesis of early enzymes was shown by the fact that DNA synthesis occurred after a culture was transferred from 44 to 30 C as late as 30 min after infection .
	manualset3
151865	2	408071	13	NULL	NULL	0	NULL	44 C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	That the infected cell at 44 C retained the capacity for synthesis of early enzymes was shown by the fact that DNA synthesis occurred after a culture was transferred from 44 to 30 C as late as 30 min after infection .
	manualset3
151866	3	408071	13	NULL	NULL	0	NULL	capacity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	That the infected cell at 44 C retained the capacity for synthesis of early enzymes was shown by the fact that DNA synthesis occurred after a culture was transferred from 44 to 30 C as late as 30 min after infection .
	manualset3
151867	4	408071	13	NULL	NULL	NULL	NULL	synthesis	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	That the infected cell at 44 C retained the capacity for synthesis of early enzymes was shown by the fact that DNA synthesis occurred after a culture was transferred from 44 to 30 C as late as 30 min after infection .
	manualset3
151868	5	408071	13	NULL	NULL	0	NULL	enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	That the infected cell at 44 C retained the capacity for synthesis of early enzymes was shown by the fact that DNA synthesis occurred after a culture was transferred from 44 to 30 C as late as 30 min after infection .
	manualset3
151869	6	408071	13	NULL	NULL	0	NULL	DNA synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	That the infected cell at 44 C retained the capacity for synthesis of early enzymes was shown by the fact that DNA synthesis occurred after a culture was transferred from 44 to 30 C as late as 30 min after infection .
	manualset3
151870	7	408071	13	NULL	NULL	0	NULL	culture	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	That the infected cell at 44 C retained the capacity for synthesis of early enzymes was shown by the fact that DNA synthesis occurred after a culture was transferred from 44 to 30 C as late as 30 min after infection .
	manualset3
151871	8	408071	13	NULL	NULL	0	NULL	44 to 30 C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	That the infected cell at 44 C retained the capacity for synthesis of early enzymes was shown by the fact that DNA synthesis occurred after a culture was transferred from 44 to 30 C as late as 30 min after infection .
	manualset3
151872	9	408071	13	NULL	NULL	0	NULL	30 min	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	That the infected cell at 44 C retained the capacity for synthesis of early enzymes was shown by the fact that DNA synthesis occurred after a culture was transferred from 44 to 30 C as late as 30 min after infection .
	manualset3
151873	10	408071	13	NULL	NULL	0	NULL	infection 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	That the infected cell at 44 C retained the capacity for synthesis of early enzymes was shown by the fact that DNA synthesis occurred after a culture was transferred from 44 to 30 C as late as 30 min after infection .
	manualset3
151874	1	408072	13	NULL	NULL	0	NULL	% ID/g	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The % ID/g in mice receiving 10 or 40 mg/kg MPTP ( 5.7 + / - 1.1 and 4.4 + / - 1.2 % / g ) was significantly lower than that in control mice ( 11.3 + / - 2.2 % / g ; P & lt ; .00001 and P & lt ; .0000001 , respectively ) .
	manualset3
151875	2	408072	13	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The % ID/g in mice receiving 10 or 40 mg/kg MPTP ( 5.7 + / - 1.1 and 4.4 + / - 1.2 % / g ) was significantly lower than that in control mice ( 11.3 + / - 2.2 % / g ; P & lt ; .00001 and P & lt ; .0000001 , respectively ) .
	manualset3
151876	3	408072	13	NULL	NULL	0	NULL	10 mg/kg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The % ID/g in mice receiving 10 or 40 mg/kg MPTP ( 5.7 + / - 1.1 and 4.4 + / - 1.2 % / g ) was significantly lower than that in control mice ( 11.3 + / - 2.2 % / g ; P & lt ; .00001 and P & lt ; .0000001 , respectively ) .
	manualset3
151877	4	408072	13	NULL	NULL	0	NULL	40 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The % ID/g in mice receiving 10 or 40 mg/kg MPTP ( 5.7 + / - 1.1 and 4.4 + / - 1.2 % / g ) was significantly lower than that in control mice ( 11.3 + / - 2.2 % / g ; P & lt ; .00001 and P & lt ; .0000001 , respectively ) .
	manualset3
151878	5	408072	13	NULL	NULL	0	NULL	MPTP 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The % ID/g in mice receiving 10 or 40 mg/kg MPTP ( 5.7 + / - 1.1 and 4.4 + / - 1.2 % / g ) was significantly lower than that in control mice ( 11.3 + / - 2.2 % / g ; P & lt ; .00001 and P & lt ; .0000001 , respectively ) .
	manualset3
151879	6	408072	13	NULL	NULL	0	NULL	5.7 + / - 1.1% / g	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The % ID/g in mice receiving 10 or 40 mg/kg MPTP ( 5.7 + / - 1.1 and 4.4 + / - 1.2 % / g ) was significantly lower than that in control mice ( 11.3 + / - 2.2 % / g ; P & lt ; .00001 and P & lt ; .0000001 , respectively ) .
	manualset3
151880	7	408072	13	NULL	NULL	0	NULL	4.4 + / - 1.2 % / g	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The % ID/g in mice receiving 10 or 40 mg/kg MPTP ( 5.7 + / - 1.1 and 4.4 + / - 1.2 % / g ) was significantly lower than that in control mice ( 11.3 + / - 2.2 % / g ; P & lt ; .00001 and P & lt ; .0000001 , respectively ) .
	manualset3
151881	8	408072	13	NULL	NULL	0	NULL	control mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The % ID/g in mice receiving 10 or 40 mg/kg MPTP ( 5.7 + / - 1.1 and 4.4 + / - 1.2 % / g ) was significantly lower than that in control mice ( 11.3 + / - 2.2 % / g ; P & lt ; .00001 and P & lt ; .0000001 , respectively ) .
	manualset3
151882	9	408072	13	NULL	NULL	0	NULL	11.3 + / - 2.2 % / g 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The % ID/g in mice receiving 10 or 40 mg/kg MPTP ( 5.7 + / - 1.1 and 4.4 + / - 1.2 % / g ) was significantly lower than that in control mice ( 11.3 + / - 2.2 % / g ; P & lt ; .00001 and P & lt ; .0000001 , respectively ) .
	manualset3
151883	10	408072	13	NULL	NULL	0	NULL	P & lt ; .00001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The % ID/g in mice receiving 10 or 40 mg/kg MPTP ( 5.7 + / - 1.1 and 4.4 + / - 1.2 % / g ) was significantly lower than that in control mice ( 11.3 + / - 2.2 % / g ; P & lt ; .00001 and P & lt ; .0000001 , respectively ) .
	manualset3
151884	11	408072	13	NULL	NULL	0	NULL	P & lt ; .0000001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The % ID/g in mice receiving 10 or 40 mg/kg MPTP ( 5.7 + / - 1.1 and 4.4 + / - 1.2 % / g ) was significantly lower than that in control mice ( 11.3 + / - 2.2 % / g ; P & lt ; .00001 and P & lt ; .0000001 , respectively ) .
	manualset3
151885	1	408073	13	NULL	NULL	0	NULL	( ( 14 ) C ) moiety 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( ( 14 ) C ) moiety from ( ( 3 ) H ) UDP ( ( 14 ) C ) glucose was incorporated by intact cotton fibers into hot water soluble , acetic-nitric reagent soluble and insoluble components , and chloroform-methanol soluble lipids ; the ( ( 3 ) H ) UDP moiety was not incorporated .
	manualset3
151886	2	408073	13	NULL	NULL	0	NULL	( ( 3 ) H ) UDP ( ( 14 ) C ) glucose 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( ( 14 ) C ) moiety from ( ( 3 ) H ) UDP ( ( 14 ) C ) glucose was incorporated by intact cotton fibers into hot water soluble , acetic-nitric reagent soluble and insoluble components , and chloroform-methanol soluble lipids ; the ( ( 3 ) H ) UDP moiety was not incorporated .
	manualset3
151887	3	408073	13	NULL	NULL	0	NULL	cotton fibers	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( ( 14 ) C ) moiety from ( ( 3 ) H ) UDP ( ( 14 ) C ) glucose was incorporated by intact cotton fibers into hot water soluble , acetic-nitric reagent soluble and insoluble components , and chloroform-methanol soluble lipids ; the ( ( 3 ) H ) UDP moiety was not incorporated .
	manualset3
151888	4	408073	13	NULL	NULL	0	NULL	hot water soluble , acetic-nitric reagent 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( ( 14 ) C ) moiety from ( ( 3 ) H ) UDP ( ( 14 ) C ) glucose was incorporated by intact cotton fibers into hot water soluble , acetic-nitric reagent soluble and insoluble components , and chloroform-methanol soluble lipids ; the ( ( 3 ) H ) UDP moiety was not incorporated .
	manualset3
151889	5	408073	13	NULL	NULL	0	NULL	soluble components	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( ( 14 ) C ) moiety from ( ( 3 ) H ) UDP ( ( 14 ) C ) glucose was incorporated by intact cotton fibers into hot water soluble , acetic-nitric reagent soluble and insoluble components , and chloroform-methanol soluble lipids ; the ( ( 3 ) H ) UDP moiety was not incorporated .
	manualset3
151890	6	408073	13	NULL	NULL	0	NULL	insoluble components	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( ( 14 ) C ) moiety from ( ( 3 ) H ) UDP ( ( 14 ) C ) glucose was incorporated by intact cotton fibers into hot water soluble , acetic-nitric reagent soluble and insoluble components , and chloroform-methanol soluble lipids ; the ( ( 3 ) H ) UDP moiety was not incorporated .
	manualset3
151891	7	408073	13	NULL	NULL	0	NULL	chloroform-methanol soluble lipids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( ( 14 ) C ) moiety from ( ( 3 ) H ) UDP ( ( 14 ) C ) glucose was incorporated by intact cotton fibers into hot water soluble , acetic-nitric reagent soluble and insoluble components , and chloroform-methanol soluble lipids ; the ( ( 3 ) H ) UDP moiety was not incorporated .
	manualset3
151892	8	408073	13	NULL	NULL	0	NULL	( ( 3 ) H ) UDP moiety 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( ( 14 ) C ) moiety from ( ( 3 ) H ) UDP ( ( 14 ) C ) glucose was incorporated by intact cotton fibers into hot water soluble , acetic-nitric reagent soluble and insoluble components , and chloroform-methanol soluble lipids ; the ( ( 3 ) H ) UDP moiety was not incorporated .
	manualset3
151893	1	408074	13	NULL	NULL	0	NULL	( 13 ) C pulsed ENDOR 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( 13 ) C pulsed ENDOR and NMR study of ( meso - ( 13 ) C-TPPFe ( OCH ( 3 ) ) ( OO ( t ) Bu ) ) ( - ) performed in this work shows that although the unpaired electron in low-spin ferrihemes containing a ROO ( - ) ligand resides in a d ( pi ) orbital at 8 K , the d ( xy ) electron configuration is favored at physiological temperatures .
	manualset3
151894	2	408074	13	NULL	NULL	0	NULL	NMR study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( 13 ) C pulsed ENDOR and NMR study of ( meso - ( 13 ) C-TPPFe ( OCH ( 3 ) ) ( OO ( t ) Bu ) ) ( - ) performed in this work shows that although the unpaired electron in low-spin ferrihemes containing a ROO ( - ) ligand resides in a d ( pi ) orbital at 8 K , the d ( xy ) electron configuration is favored at physiological temperatures .
	manualset3
151895	3	408074	13	NULL	NULL	0	NULL	( meso - ( 13 ) C-TPPFe ( OCH ( 3 ) ) ( OO ( t ) Bu ) ) ( - ) 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( 13 ) C pulsed ENDOR and NMR study of ( meso - ( 13 ) C-TPPFe ( OCH ( 3 ) ) ( OO ( t ) Bu ) ) ( - ) performed in this work shows that although the unpaired electron in low-spin ferrihemes containing a ROO ( - ) ligand resides in a d ( pi ) orbital at 8 K , the d ( xy ) electron configuration is favored at physiological temperatures .
	manualset3
151896	4	408074	13	NULL	NULL	0	NULL	work 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( 13 ) C pulsed ENDOR and NMR study of ( meso - ( 13 ) C-TPPFe ( OCH ( 3 ) ) ( OO ( t ) Bu ) ) ( - ) performed in this work shows that although the unpaired electron in low-spin ferrihemes containing a ROO ( - ) ligand resides in a d ( pi ) orbital at 8 K , the d ( xy ) electron configuration is favored at physiological temperatures .
	manualset3
151897	5	408074	13	NULL	NULL	0	NULL	electron	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( 13 ) C pulsed ENDOR and NMR study of ( meso - ( 13 ) C-TPPFe ( OCH ( 3 ) ) ( OO ( t ) Bu ) ) ( - ) performed in this work shows that although the unpaired electron in low-spin ferrihemes containing a ROO ( - ) ligand resides in a d ( pi ) orbital at 8 K , the d ( xy ) electron configuration is favored at physiological temperatures .
	manualset3
151898	6	408074	13	NULL	NULL	0	NULL	low-spin ferrihemes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( 13 ) C pulsed ENDOR and NMR study of ( meso - ( 13 ) C-TPPFe ( OCH ( 3 ) ) ( OO ( t ) Bu ) ) ( - ) performed in this work shows that although the unpaired electron in low-spin ferrihemes containing a ROO ( - ) ligand resides in a d ( pi ) orbital at 8 K , the d ( xy ) electron configuration is favored at physiological temperatures .
	manualset3
151899	7	408074	13	NULL	NULL	0	NULL	ROO ( - ) ligand	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( 13 ) C pulsed ENDOR and NMR study of ( meso - ( 13 ) C-TPPFe ( OCH ( 3 ) ) ( OO ( t ) Bu ) ) ( - ) performed in this work shows that although the unpaired electron in low-spin ferrihemes containing a ROO ( - ) ligand resides in a d ( pi ) orbital at 8 K , the d ( xy ) electron configuration is favored at physiological temperatures .
	manualset3
151900	8	408074	13	NULL	NULL	0	NULL	d ( pi ) orbital	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( 13 ) C pulsed ENDOR and NMR study of ( meso - ( 13 ) C-TPPFe ( OCH ( 3 ) ) ( OO ( t ) Bu ) ) ( - ) performed in this work shows that although the unpaired electron in low-spin ferrihemes containing a ROO ( - ) ligand resides in a d ( pi ) orbital at 8 K , the d ( xy ) electron configuration is favored at physiological temperatures .
	manualset3
151901	9	408074	13	NULL	NULL	0	NULL	8 K	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( 13 ) C pulsed ENDOR and NMR study of ( meso - ( 13 ) C-TPPFe ( OCH ( 3 ) ) ( OO ( t ) Bu ) ) ( - ) performed in this work shows that although the unpaired electron in low-spin ferrihemes containing a ROO ( - ) ligand resides in a d ( pi ) orbital at 8 K , the d ( xy ) electron configuration is favored at physiological temperatures .
	manualset3
151902	10	408074	13	NULL	NULL	0	NULL	d ( xy ) electron configuration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( 13 ) C pulsed ENDOR and NMR study of ( meso - ( 13 ) C-TPPFe ( OCH ( 3 ) ) ( OO ( t ) Bu ) ) ( - ) performed in this work shows that although the unpaired electron in low-spin ferrihemes containing a ROO ( - ) ligand resides in a d ( pi ) orbital at 8 K , the d ( xy ) electron configuration is favored at physiological temperatures .
	manualset3
151903	11	408074	13	NULL	NULL	0	NULL	physiological temperatures	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( 13 ) C pulsed ENDOR and NMR study of ( meso - ( 13 ) C-TPPFe ( OCH ( 3 ) ) ( OO ( t ) Bu ) ) ( - ) performed in this work shows that although the unpaired electron in low-spin ferrihemes containing a ROO ( - ) ligand resides in a d ( pi ) orbital at 8 K , the d ( xy ) electron configuration is favored at physiological temperatures .
	manualset3
151904	1	408075	13	NULL	NULL	0	NULL	( 3H ) 20-COOH-AA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( 3H ) 20-COOH-AA accumulated primarily in the culture medium , together with additional radiolabeled metabolites identified as the chain-shortened dicarboxylic acids 18-COOH-18 : 4 , 18-COOH-18 : 3 , and 16-COOH-16 : 3 .
	manualset3
151905	2	408075	13	NULL	NULL	0	NULL	culture medium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( 3H ) 20-COOH-AA accumulated primarily in the culture medium , together with additional radiolabeled metabolites identified as the chain-shortened dicarboxylic acids 18-COOH-18 : 4 , 18-COOH-18 : 3 , and 16-COOH-16 : 3 .
	manualset3
151906	3	408075	13	NULL	NULL	0	NULL	metabolites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( 3H ) 20-COOH-AA accumulated primarily in the culture medium , together with additional radiolabeled metabolites identified as the chain-shortened dicarboxylic acids 18-COOH-18 : 4 , 18-COOH-18 : 3 , and 16-COOH-16 : 3 .
	manualset3
151907	4	408075	13	NULL	NULL	0	NULL	chain-shortened dicarboxylic acids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( 3H ) 20-COOH-AA accumulated primarily in the culture medium , together with additional radiolabeled metabolites identified as the chain-shortened dicarboxylic acids 18-COOH-18 : 4 , 18-COOH-18 : 3 , and 16-COOH-16 : 3 .
	manualset3
151908	5	408075	13	NULL	NULL	0	NULL	18-COOH-18 : 4	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( 3H ) 20-COOH-AA accumulated primarily in the culture medium , together with additional radiolabeled metabolites identified as the chain-shortened dicarboxylic acids 18-COOH-18 : 4 , 18-COOH-18 : 3 , and 16-COOH-16 : 3 .
	manualset3
151909	6	408075	13	NULL	NULL	0	NULL	18-COOH-18 : 3	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( 3H ) 20-COOH-AA accumulated primarily in the culture medium , together with additional radiolabeled metabolites identified as the chain-shortened dicarboxylic acids 18-COOH-18 : 4 , 18-COOH-18 : 3 , and 16-COOH-16 : 3 .
	manualset3
151910	7	408075	13	NULL	NULL	0	NULL	16-COOH-16 : 3 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( 3H ) 20-COOH-AA accumulated primarily in the culture medium , together with additional radiolabeled metabolites identified as the chain-shortened dicarboxylic acids 18-COOH-18 : 4 , 18-COOH-18 : 3 , and 16-COOH-16 : 3 .
	manualset3
151911	1	408076	13	NULL	NULL	0	NULL	 ( 3H ) iditol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( 3H ) iditol was readily converted to ( 3H ) sorbose by the stereospecific enzyme , L-iditol dehydrogenase , indicating that it originated from Ins-3 , 4 , 5 , 6 - P4 .
	manualset3
151912	2	408076	13	NULL	NULL	0	NULL	( 3H ) sorbose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( 3H ) iditol was readily converted to ( 3H ) sorbose by the stereospecific enzyme , L-iditol dehydrogenase , indicating that it originated from Ins-3 , 4 , 5 , 6 - P4 .
	manualset3
151913	3	408076	13	NULL	NULL	0	NULL	stereospecific enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( 3H ) iditol was readily converted to ( 3H ) sorbose by the stereospecific enzyme , L-iditol dehydrogenase , indicating that it originated from Ins-3 , 4 , 5 , 6 - P4 .
	manualset3
151914	4	408076	13	NULL	NULL	0	NULL	L-iditol dehydrogenase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( 3H ) iditol was readily converted to ( 3H ) sorbose by the stereospecific enzyme , L-iditol dehydrogenase , indicating that it originated from Ins-3 , 4 , 5 , 6 - P4 .
	manualset3
151915	5	408076	13	NULL	NULL	0	NULL	Ins-3 , 4 , 5 , 6 - P4	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ( 3H ) iditol was readily converted to ( 3H ) sorbose by the stereospecific enzyme , L-iditol dehydrogenase , indicating that it originated from Ins-3 , 4 , 5 , 6 - P4 .
	manualset3
151916	1	408077	13	NULL	NULL	0	NULL	0.1-Hz oscillation 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 0.1-Hz oscillation at a green light wavelength of 546 nm exhibits greater amplitude in arteries than in veins and is primarily caused by vasomotion , whereas the 0.1-Hz oscillation at a red light wavelength of 630 nm exhibits greater amplitude in veins than in arteries and is primarily caused by changes of deoxyhemoglobin concentration .
	manualset3
151917	2	408077	13	NULL	NULL	0	NULL	green light wavelength	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 0.1-Hz oscillation at a green light wavelength of 546 nm exhibits greater amplitude in arteries than in veins and is primarily caused by vasomotion , whereas the 0.1-Hz oscillation at a red light wavelength of 630 nm exhibits greater amplitude in veins than in arteries and is primarily caused by changes of deoxyhemoglobin concentration .
	manualset3
151918	3	408077	13	NULL	NULL	0	NULL	546 nm 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 0.1-Hz oscillation at a green light wavelength of 546 nm exhibits greater amplitude in arteries than in veins and is primarily caused by vasomotion , whereas the 0.1-Hz oscillation at a red light wavelength of 630 nm exhibits greater amplitude in veins than in arteries and is primarily caused by changes of deoxyhemoglobin concentration .
	manualset3
151919	4	408077	13	NULL	NULL	0	NULL	amplitude	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 0.1-Hz oscillation at a green light wavelength of 546 nm exhibits greater amplitude in arteries than in veins and is primarily caused by vasomotion , whereas the 0.1-Hz oscillation at a red light wavelength of 630 nm exhibits greater amplitude in veins than in arteries and is primarily caused by changes of deoxyhemoglobin concentration .
	manualset3
151920	5	408077	13	NULL	NULL	0	NULL	arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The 0.1-Hz oscillation at a green light wavelength of 546 nm exhibits greater amplitude in arteries than in veins and is primarily caused by vasomotion , whereas the 0.1-Hz oscillation at a red light wavelength of 630 nm exhibits greater amplitude in veins than in arteries and is primarily caused by changes of deoxyhemoglobin concentration .
	manualset3
151921	6	408077	13	NULL	NULL	0	NULL	veins 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The 0.1-Hz oscillation at a green light wavelength of 546 nm exhibits greater amplitude in arteries than in veins and is primarily caused by vasomotion , whereas the 0.1-Hz oscillation at a red light wavelength of 630 nm exhibits greater amplitude in veins than in arteries and is primarily caused by changes of deoxyhemoglobin concentration .
	manualset3
151922	7	408077	13	NULL	NULL	0	NULL	vasomotion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 0.1-Hz oscillation at a green light wavelength of 546 nm exhibits greater amplitude in arteries than in veins and is primarily caused by vasomotion , whereas the 0.1-Hz oscillation at a red light wavelength of 630 nm exhibits greater amplitude in veins than in arteries and is primarily caused by changes of deoxyhemoglobin concentration .
	manualset3
151923	8	408077	13	NULL	NULL	0	NULL	0.1-Hz oscillation	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 0.1-Hz oscillation at a green light wavelength of 546 nm exhibits greater amplitude in arteries than in veins and is primarily caused by vasomotion , whereas the 0.1-Hz oscillation at a red light wavelength of 630 nm exhibits greater amplitude in veins than in arteries and is primarily caused by changes of deoxyhemoglobin concentration .
	manualset3
151924	9	408077	13	NULL	NULL	0	NULL	red light wavelength 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 0.1-Hz oscillation at a green light wavelength of 546 nm exhibits greater amplitude in arteries than in veins and is primarily caused by vasomotion , whereas the 0.1-Hz oscillation at a red light wavelength of 630 nm exhibits greater amplitude in veins than in arteries and is primarily caused by changes of deoxyhemoglobin concentration .
	manualset3
151925	10	408077	13	NULL	NULL	0	NULL	630 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 0.1-Hz oscillation at a green light wavelength of 546 nm exhibits greater amplitude in arteries than in veins and is primarily caused by vasomotion , whereas the 0.1-Hz oscillation at a red light wavelength of 630 nm exhibits greater amplitude in veins than in arteries and is primarily caused by changes of deoxyhemoglobin concentration .
	manualset3
151926	11	408077	13	NULL	NULL	0	NULL	 amplitude	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 0.1-Hz oscillation at a green light wavelength of 546 nm exhibits greater amplitude in arteries than in veins and is primarily caused by vasomotion , whereas the 0.1-Hz oscillation at a red light wavelength of 630 nm exhibits greater amplitude in veins than in arteries and is primarily caused by changes of deoxyhemoglobin concentration .
	manualset3
151927	12	408077	13	NULL	NULL	0	NULL	veins	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The 0.1-Hz oscillation at a green light wavelength of 546 nm exhibits greater amplitude in arteries than in veins and is primarily caused by vasomotion , whereas the 0.1-Hz oscillation at a red light wavelength of 630 nm exhibits greater amplitude in veins than in arteries and is primarily caused by changes of deoxyhemoglobin concentration .
	manualset3
151928	13	408077	13	NULL	NULL	0	NULL	arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The 0.1-Hz oscillation at a green light wavelength of 546 nm exhibits greater amplitude in arteries than in veins and is primarily caused by vasomotion , whereas the 0.1-Hz oscillation at a red light wavelength of 630 nm exhibits greater amplitude in veins than in arteries and is primarily caused by changes of deoxyhemoglobin concentration .
	manualset3
151929	14	408077	13	NULL	NULL	0	NULL	changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 0.1-Hz oscillation at a green light wavelength of 546 nm exhibits greater amplitude in arteries than in veins and is primarily caused by vasomotion , whereas the 0.1-Hz oscillation at a red light wavelength of 630 nm exhibits greater amplitude in veins than in arteries and is primarily caused by changes of deoxyhemoglobin concentration .
	manualset3
151930	15	408077	13	NULL	NULL	0	NULL	deoxyhemoglobin concentration 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The 0.1-Hz oscillation at a green light wavelength of 546 nm exhibits greater amplitude in arteries than in veins and is primarily caused by vasomotion , whereas the 0.1-Hz oscillation at a red light wavelength of 630 nm exhibits greater amplitude in veins than in arteries and is primarily caused by changes of deoxyhemoglobin concentration .
	manualset3
151931	16	408077	13	NULL	NULL	0	NULL	exhibits	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 0.1-Hz oscillation at a green light wavelength of 546 nm exhibits greater amplitude in arteries than in veins and is primarily caused by vasomotion , whereas the 0.1-Hz oscillation at a red light wavelength of 630 nm exhibits greater amplitude in veins than in arteries and is primarily caused by changes of deoxyhemoglobin concentration .
	manualset3
151932	1	408078	13	NULL	NULL	0	NULL	quantitative test	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A quantitative test for chemosensitivity of short-term cultures of human lymphomas .
	manualset3
151933	2	408078	13	NULL	NULL	0	NULL	chemosensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A quantitative test for chemosensitivity of short-term cultures of human lymphomas .
	manualset3
151934	3	408078	13	NULL	NULL	0	NULL	 cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A quantitative test for chemosensitivity of short-term cultures of human lymphomas .
	manualset3
151935	4	408078	13	NULL	NULL	0	NULL	 human lymphomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A quantitative test for chemosensitivity of short-term cultures of human lymphomas .
	manualset3
151936	1	408079	13	NULL	NULL	0	NULL	0.7 M NaCl fraction 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 0.7 M NaCl fraction showed an electrophoretic mobility in polyacrylamide gel identical to that of type II collagen , CNBr-derived peptides very similar to type II collagen CNBr-peptides , and a reaggregation behavior closely related to type II collagen as observed by electron microscopy .
	manualset3
151937	2	408079	13	NULL	NULL	0	NULL	electrophoretic mobility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 0.7 M NaCl fraction showed an electrophoretic mobility in polyacrylamide gel identical to that of type II collagen , CNBr-derived peptides very similar to type II collagen CNBr-peptides , and a reaggregation behavior closely related to type II collagen as observed by electron microscopy .
	manualset3
151938	3	408079	13	NULL	NULL	0	NULL	polyacrylamide gel	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The 0.7 M NaCl fraction showed an electrophoretic mobility in polyacrylamide gel identical to that of type II collagen , CNBr-derived peptides very similar to type II collagen CNBr-peptides , and a reaggregation behavior closely related to type II collagen as observed by electron microscopy .
	manualset3
151939	4	408079	13	NULL	NULL	0	NULL	type II collagen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The 0.7 M NaCl fraction showed an electrophoretic mobility in polyacrylamide gel identical to that of type II collagen , CNBr-derived peptides very similar to type II collagen CNBr-peptides , and a reaggregation behavior closely related to type II collagen as observed by electron microscopy .
	manualset3
151940	5	408079	13	NULL	NULL	0	NULL	CNBr-derived peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The 0.7 M NaCl fraction showed an electrophoretic mobility in polyacrylamide gel identical to that of type II collagen , CNBr-derived peptides very similar to type II collagen CNBr-peptides , and a reaggregation behavior closely related to type II collagen as observed by electron microscopy .
	manualset3
151941	6	408079	13	NULL	NULL	0	NULL	type II collagen CNBr-peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The 0.7 M NaCl fraction showed an electrophoretic mobility in polyacrylamide gel identical to that of type II collagen , CNBr-derived peptides very similar to type II collagen CNBr-peptides , and a reaggregation behavior closely related to type II collagen as observed by electron microscopy .
	manualset3
151942	7	408079	13	NULL	NULL	0	NULL	 reaggregation behavior	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 0.7 M NaCl fraction showed an electrophoretic mobility in polyacrylamide gel identical to that of type II collagen , CNBr-derived peptides very similar to type II collagen CNBr-peptides , and a reaggregation behavior closely related to type II collagen as observed by electron microscopy .
	manualset3
151943	8	408079	13	NULL	NULL	0	NULL	type II collagen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The 0.7 M NaCl fraction showed an electrophoretic mobility in polyacrylamide gel identical to that of type II collagen , CNBr-derived peptides very similar to type II collagen CNBr-peptides , and a reaggregation behavior closely related to type II collagen as observed by electron microscopy .
	manualset3
151944	9	408079	13	NULL	NULL	0	NULL	electron microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The 0.7 M NaCl fraction showed an electrophoretic mobility in polyacrylamide gel identical to that of type II collagen , CNBr-derived peptides very similar to type II collagen CNBr-peptides , and a reaggregation behavior closely related to type II collagen as observed by electron microscopy .
	manualset3
151945	1	408080	13	NULL	NULL	0	NULL	1-N-oxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1-N-oxide differs from the parent compound by its toxic effect on HeLa cells ( ID50 = 5.0 ppm ) reflected primarily through cellular vacuole formation from dilation of rough endoplasmic reticulum structures .
	manualset3
151946	2	408080	13	NULL	NULL	0	NULL	parent compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1-N-oxide differs from the parent compound by its toxic effect on HeLa cells ( ID50 = 5.0 ppm ) reflected primarily through cellular vacuole formation from dilation of rough endoplasmic reticulum structures .
	manualset3
151947	3	408080	13	NULL	NULL	0	NULL	toxic effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1-N-oxide differs from the parent compound by its toxic effect on HeLa cells ( ID50 = 5.0 ppm ) reflected primarily through cellular vacuole formation from dilation of rough endoplasmic reticulum structures .
	manualset3
151948	4	408080	13	NULL	NULL	0	NULL	HeLa cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1-N-oxide differs from the parent compound by its toxic effect on HeLa cells ( ID50 = 5.0 ppm ) reflected primarily through cellular vacuole formation from dilation of rough endoplasmic reticulum structures .
	manualset3
151949	5	408080	13	NULL	NULL	0	NULL	ID50 = 5.0 ppm 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1-N-oxide differs from the parent compound by its toxic effect on HeLa cells ( ID50 = 5.0 ppm ) reflected primarily through cellular vacuole formation from dilation of rough endoplasmic reticulum structures .
	manualset3
151950	6	408080	13	NULL	NULL	0	NULL	cellular vacuole formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1-N-oxide differs from the parent compound by its toxic effect on HeLa cells ( ID50 = 5.0 ppm ) reflected primarily through cellular vacuole formation from dilation of rough endoplasmic reticulum structures .
	manualset3
151951	7	408080	13	NULL	NULL	0	NULL	dilation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1-N-oxide differs from the parent compound by its toxic effect on HeLa cells ( ID50 = 5.0 ppm ) reflected primarily through cellular vacuole formation from dilation of rough endoplasmic reticulum structures .
	manualset3
151952	8	408080	13	NULL	NULL	0	NULL	rough endoplasmic reticulum structures	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1-N-oxide differs from the parent compound by its toxic effect on HeLa cells ( ID50 = 5.0 ppm ) reflected primarily through cellular vacuole formation from dilation of rough endoplasmic reticulum structures .
	manualset3
151953	1	408081	13	NULL	NULL	0	NULL	1.5-Mb region	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1.5-Mb region spanning the myotonic dystrophy locus shows uniform recombination frequency .
	manualset3
151954	2	408081	13	NULL	NULL	0	NULL	myotonic dystrophy locus	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1.5-Mb region spanning the myotonic dystrophy locus shows uniform recombination frequency .
	manualset3
151955	3	408081	13	NULL	NULL	0	NULL	uniform recombination frequency	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1.5-Mb region spanning the myotonic dystrophy locus shows uniform recombination frequency .
	manualset3
151956	1	408082	13	NULL	NULL	0	NULL	10-fold 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 10-fold derepression of secA expression by protein export defects was at the translational level since no further increases in gene X or secA mRNA levels were detected during this period , and a secA-lacZ protein fusion but not an operon fusion was appropriately derepressed .
	manualset3
151957	2	408082	13	NULL	NULL	0	NULL	derepression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 10-fold derepression of secA expression by protein export defects was at the translational level since no further increases in gene X or secA mRNA levels were detected during this period , and a secA-lacZ protein fusion but not an operon fusion was appropriately derepressed .
	manualset3
151958	3	408082	13	NULL	NULL	0	NULL	secA expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 10-fold derepression of secA expression by protein export defects was at the translational level since no further increases in gene X or secA mRNA levels were detected during this period , and a secA-lacZ protein fusion but not an operon fusion was appropriately derepressed .
	manualset3
151959	4	408082	13	NULL	NULL	0	NULL	protein export defects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 10-fold derepression of secA expression by protein export defects was at the translational level since no further increases in gene X or secA mRNA levels were detected during this period , and a secA-lacZ protein fusion but not an operon fusion was appropriately derepressed .
	manualset3
151960	5	408082	13	NULL	NULL	0	NULL	translational level 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 10-fold derepression of secA expression by protein export defects was at the translational level since no further increases in gene X or secA mRNA levels were detected during this period , and a secA-lacZ protein fusion but not an operon fusion was appropriately derepressed .
	manualset3
151961	6	408082	13	NULL	NULL	0	NULL	increases	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 10-fold derepression of secA expression by protein export defects was at the translational level since no further increases in gene X or secA mRNA levels were detected during this period , and a secA-lacZ protein fusion but not an operon fusion was appropriately derepressed .
	manualset3
151962	7	408082	13	NULL	NULL	0	NULL	 gene X mRNA levels	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The 10-fold derepression of secA expression by protein export defects was at the translational level since no further increases in gene X or secA mRNA levels were detected during this period , and a secA-lacZ protein fusion but not an operon fusion was appropriately derepressed .
	manualset3
151963	8	408082	13	NULL	NULL	0	NULL	secA mRNA levels	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The 10-fold derepression of secA expression by protein export defects was at the translational level since no further increases in gene X or secA mRNA levels were detected during this period , and a secA-lacZ protein fusion but not an operon fusion was appropriately derepressed .
	manualset3
151964	9	408082	13	NULL	NULL	0	NULL	period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The 10-fold derepression of secA expression by protein export defects was at the translational level since no further increases in gene X or secA mRNA levels were detected during this period , and a secA-lacZ protein fusion but not an operon fusion was appropriately derepressed .
	manualset3
151965	10	408082	13	NULL	NULL	0	NULL	secA-lacZ protein fusion	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The 10-fold derepression of secA expression by protein export defects was at the translational level since no further increases in gene X or secA mRNA levels were detected during this period , and a secA-lacZ protein fusion but not an operon fusion was appropriately derepressed .
	manualset3
151966	11	408082	13	NULL	NULL	0	NULL	operon fusion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 10-fold derepression of secA expression by protein export defects was at the translational level since no further increases in gene X or secA mRNA levels were detected during this period , and a secA-lacZ protein fusion but not an operon fusion was appropriately derepressed .
	manualset3
151967	1	408083	13	NULL	NULL	0	NULL	100-ms deflections 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 100-ms deflections of AEFs were higher in amplitude and shorter in latency to contra - than ipsilateral stimuli ; a similar behavior was seen in the tangential source components of AEPs .
	manualset3
151968	2	408083	13	NULL	NULL	0	NULL	AEFs	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 100-ms deflections of AEFs were higher in amplitude and shorter in latency to contra - than ipsilateral stimuli ; a similar behavior was seen in the tangential source components of AEPs .
	manualset3
151969	3	408083	13	NULL	NULL	0	NULL	amplitude	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 100-ms deflections of AEFs were higher in amplitude and shorter in latency to contra - than ipsilateral stimuli ; a similar behavior was seen in the tangential source components of AEPs .
	manualset3
151970	4	408083	13	NULL	NULL	0	NULL	 latency 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 100-ms deflections of AEFs were higher in amplitude and shorter in latency to contra - than ipsilateral stimuli ; a similar behavior was seen in the tangential source components of AEPs .
	manualset3
151971	5	408083	13	NULL	NULL	0	NULL	ipsilateral stimuli	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 100-ms deflections of AEFs were higher in amplitude and shorter in latency to contra - than ipsilateral stimuli ; a similar behavior was seen in the tangential source components of AEPs .
	manualset3
151972	6	408083	13	NULL	NULL	0	NULL	behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 100-ms deflections of AEFs were higher in amplitude and shorter in latency to contra - than ipsilateral stimuli ; a similar behavior was seen in the tangential source components of AEPs .
	manualset3
151973	7	408083	13	NULL	NULL	0	NULL	tangential source components	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The 100-ms deflections of AEFs were higher in amplitude and shorter in latency to contra - than ipsilateral stimuli ; a similar behavior was seen in the tangential source components of AEPs .
	manualset3
151974	8	408083	13	NULL	NULL	0	NULL	AEPs	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 100-ms deflections of AEFs were higher in amplitude and shorter in latency to contra - than ipsilateral stimuli ; a similar behavior was seen in the tangential source components of AEPs .
	manualset3
151979	1	408084	13	NULL	NULL	0	NULL	11	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The 11 Virginia barrier islands are undergoing rapid changes in shore-line configuration .
	manualset3
151980	2	408084	13	NULL	NULL	0	NULL	Virginia barrier islands	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The 11 Virginia barrier islands are undergoing rapid changes in shore-line configuration .
	manualset3
151982	3	408084	13	NULL	NULL	0	NULL	changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 11 Virginia barrier islands are undergoing rapid changes in shore-line configuration .
	manualset3
151983	4	408084	13	NULL	NULL	0	NULL	shore-line configuration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 11 Virginia barrier islands are undergoing rapid changes in shore-line configuration .
	manualset3
151984	1	408085	13	NULL	NULL	0	NULL	111In-T101	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The 111In-T101 rapidly distributed throughout the regional lymphatic compartment and passed into the systemic circulation .
	manualset3
151985	2	408085	13	NULL	NULL	0	NULL	regional lymphatic compartment	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The 111In-T101 rapidly distributed throughout the regional lymphatic compartment and passed into the systemic circulation .
	manualset3
151986	3	408085	13	NULL	NULL	0	NULL	systemic circulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 111In-T101 rapidly distributed throughout the regional lymphatic compartment and passed into the systemic circulation .
	manualset3
151987	1	408086	13	NULL	NULL	0	NULL	13C-acetate breath tests 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The 13C-acetate and - octanoate breath tests represent an alternative to this method , which has been extensively validated .
	manualset3
151988	2	408086	13	NULL	NULL	0	NULL	13C- octanoate breath tests	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The 13C-acetate and - octanoate breath tests represent an alternative to this method , which has been extensively validated .
	manualset3
151989	4	408086	13	NULL	NULL	NULL	NULL	 method 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The 13C-acetate and - octanoate breath tests represent an alternative to this method , which has been extensively validated .
	manualset3
151990	3	408086	13	NULL	NULL	0	NULL	alternative	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 13C-acetate and - octanoate breath tests represent an alternative to this method , which has been extensively validated .
	manualset3
151991	1	408087	13	NULL	NULL	0	NULL	16 nm periodicity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 16 nm periodicity visible in some negatively stained specimens ( caused by the pairing of cooperatively bound kinesin dimers ) is not detected by surface shadowing .
	manualset3
151992	2	408087	13	NULL	NULL	0	NULL	specimens	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The 16 nm periodicity visible in some negatively stained specimens ( caused by the pairing of cooperatively bound kinesin dimers ) is not detected by surface shadowing .
	manualset3
151993	3	408087	13	NULL	NULL	0	NULL	pairing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 16 nm periodicity visible in some negatively stained specimens ( caused by the pairing of cooperatively bound kinesin dimers ) is not detected by surface shadowing .
	manualset3
151994	4	408087	13	NULL	NULL	0	NULL	kinesin dimers 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The 16 nm periodicity visible in some negatively stained specimens ( caused by the pairing of cooperatively bound kinesin dimers ) is not detected by surface shadowing .
	manualset3
151995	5	408087	13	NULL	NULL	0	NULL	surface shadowing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 16 nm periodicity visible in some negatively stained specimens ( caused by the pairing of cooperatively bound kinesin dimers ) is not detected by surface shadowing .
	manualset3
151997	1	408088	13	NULL	NULL	0	NULL	questionnaire	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A questionnaire was also completed for each of the subjects , to test their perception of urinary schistosomiasis and its transmission .
	manualset3
151999	2	408088	13	NULL	NULL	0	NULL	subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A questionnaire was also completed for each of the subjects , to test their perception of urinary schistosomiasis and its transmission .
	manualset3
152000	3	408088	13	NULL	NULL	0	NULL	perception 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A questionnaire was also completed for each of the subjects , to test their perception of urinary schistosomiasis and its transmission .
	manualset3
152001	4	408088	13	NULL	NULL	0	NULL	urinary schistosomiasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A questionnaire was also completed for each of the subjects , to test their perception of urinary schistosomiasis and its transmission .
	manualset3
152002	5	408088	13	NULL	NULL	0	NULL	transmission 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A questionnaire was also completed for each of the subjects , to test their perception of urinary schistosomiasis and its transmission .
	manualset3
152003	1	408089	13	NULL	NULL	0	NULL	1611-base-pair gene termination codon	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1611-base-pair gene termination codon overlaps the initiator ATG of the sopI gene , which encodes the sensory rhodopsin I apoprotein .
	manualset3
152004	2	408089	13	NULL	NULL	0	NULL	initiator ATG	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1611-base-pair gene termination codon overlaps the initiator ATG of the sopI gene , which encodes the sensory rhodopsin I apoprotein .
	manualset3
152005	3	408089	13	NULL	NULL	0	NULL	sopI gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1611-base-pair gene termination codon overlaps the initiator ATG of the sopI gene , which encodes the sensory rhodopsin I apoprotein .
	manualset3
152006	4	408089	13	NULL	NULL	0	NULL	sensory rhodopsin I apoprotein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1611-base-pair gene termination codon overlaps the initiator ATG of the sopI gene , which encodes the sensory rhodopsin I apoprotein .
	manualset3
152011	1	408090	13	NULL	NULL	0	NULL	169G ) A substitution ( A57T )	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 169G ) A substitution ( A57T ) appears to be a polymorphism ( 4 patients , 7.4 % ) .
	manualset3
152012	2	408090	13	NULL	NULL	0	NULL	polymorphism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 169G ) A substitution ( A57T ) appears to be a polymorphism ( 4 patients , 7.4 % ) .
	manualset3
152013	3	408090	13	NULL	NULL	0	NULL	4 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The 169G ) A substitution ( A57T ) appears to be a polymorphism ( 4 patients , 7.4 % ) .
	manualset3
152014	4	408090	13	NULL	NULL	0	NULL	 7.4 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 169G ) A substitution ( A57T ) appears to be a polymorphism ( 4 patients , 7.4 % ) .
	manualset3
152017	1	408091	13	NULL	NULL	0	NULL	16S rRNA gene sequence 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The 16S rRNA gene sequence similarity between strain S5-5 ( T ) and members of the genus Roseivivax was in the range 95.0-96 .7 % .
	manualset3
152018	2	408091	13	NULL	NULL	0	NULL	similarity 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The 16S rRNA gene sequence similarity between strain S5-5 ( T ) and members of the genus Roseivivax was in the range 95.0-96 .7 % .
	manualset3
152019	3	408091	13	NULL	NULL	0	NULL	strain S5-5 ( T ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The 16S rRNA gene sequence similarity between strain S5-5 ( T ) and members of the genus Roseivivax was in the range 95.0-96 .7 % .
	manualset3
152021	4	408091	13	NULL	NULL	0	NULL	members	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The 16S rRNA gene sequence similarity between strain S5-5 ( T ) and members of the genus Roseivivax was in the range 95.0-96 .7 % .
	manualset3
152022	5	408091	13	NULL	NULL	0	NULL	genus Roseivivax	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The 16S rRNA gene sequence similarity between strain S5-5 ( T ) and members of the genus Roseivivax was in the range 95.0-96 .7 % .
	manualset3
152023	6	408091	13	NULL	NULL	0	NULL	range 95.0-96 .7 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 16S rRNA gene sequence similarity between strain S5-5 ( T ) and members of the genus Roseivivax was in the range 95.0-96 .7 % .
	manualset3
152027	1	408092	13	NULL	NULL	0	NULL	17 X 8-hydroxylase activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 17 X 8-hydroxylase activities were found to be low in liver microsomes from individuals possessing the deletion or mutations in the CYP2A6 gene .
	manualset3
152028	2	408092	13	NULL	NULL	0	NULL	liver microsomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The 17 X 8-hydroxylase activities were found to be low in liver microsomes from individuals possessing the deletion or mutations in the CYP2A6 gene .
	manualset3
152030	3	408092	13	NULL	NULL	0	NULL	individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The 17 X 8-hydroxylase activities were found to be low in liver microsomes from individuals possessing the deletion or mutations in the CYP2A6 gene .
	manualset3
152031	4	408092	13	NULL	NULL	0	NULL	deletion 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 17 X 8-hydroxylase activities were found to be low in liver microsomes from individuals possessing the deletion or mutations in the CYP2A6 gene .
	manualset3
152033	5	408092	13	NULL	NULL	0	NULL	mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 17 X 8-hydroxylase activities were found to be low in liver microsomes from individuals possessing the deletion or mutations in the CYP2A6 gene .
	manualset3
152034	6	408092	13	NULL	NULL	0	NULL	CYP2A6 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The 17 X 8-hydroxylase activities were found to be low in liver microsomes from individuals possessing the deletion or mutations in the CYP2A6 gene .
	manualset3
152035	1	408093	13	NULL	NULL	0	NULL	18S RNA-B-infected dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The 18S RNA-B-infected dogs suffered from hypochloremia ( 8 ) , hyponatremia ( 6 ) , hypernatremia ( 2 ) and increase in blood pH ( 10 ) .
	manualset3
152036	2	408093	13	NULL	NULL	0	NULL	hypochloremia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The 18S RNA-B-infected dogs suffered from hypochloremia ( 8 ) , hyponatremia ( 6 ) , hypernatremia ( 2 ) and increase in blood pH ( 10 ) .
	manualset3
152037	3	408093	13	NULL	NULL	0	NULL	8	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The 18S RNA-B-infected dogs suffered from hypochloremia ( 8 ) , hyponatremia ( 6 ) , hypernatremia ( 2 ) and increase in blood pH ( 10 ) .
	manualset3
152038	4	408093	13	NULL	NULL	0	NULL	hyponatremia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The 18S RNA-B-infected dogs suffered from hypochloremia ( 8 ) , hyponatremia ( 6 ) , hypernatremia ( 2 ) and increase in blood pH ( 10 ) .
	manualset3
152039	5	408093	13	NULL	NULL	0	NULL	6	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The 18S RNA-B-infected dogs suffered from hypochloremia ( 8 ) , hyponatremia ( 6 ) , hypernatremia ( 2 ) and increase in blood pH ( 10 ) .
	manualset3
152040	6	408093	13	NULL	NULL	0	NULL	hypernatremia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The 18S RNA-B-infected dogs suffered from hypochloremia ( 8 ) , hyponatremia ( 6 ) , hypernatremia ( 2 ) and increase in blood pH ( 10 ) .
	manualset3
152041	7	408093	13	NULL	NULL	0	NULL	 2 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The 18S RNA-B-infected dogs suffered from hypochloremia ( 8 ) , hyponatremia ( 6 ) , hypernatremia ( 2 ) and increase in blood pH ( 10 ) .
	manualset3
152042	8	408093	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 18S RNA-B-infected dogs suffered from hypochloremia ( 8 ) , hyponatremia ( 6 ) , hypernatremia ( 2 ) and increase in blood pH ( 10 ) .
	manualset3
152043	9	408093	13	NULL	NULL	0	NULL	blood pH	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The 18S RNA-B-infected dogs suffered from hypochloremia ( 8 ) , hyponatremia ( 6 ) , hypernatremia ( 2 ) and increase in blood pH ( 10 ) .
	manualset3
152044	10	408093	13	NULL	NULL	0	NULL	10	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The 18S RNA-B-infected dogs suffered from hypochloremia ( 8 ) , hyponatremia ( 6 ) , hypernatremia ( 2 ) and increase in blood pH ( 10 ) .
	manualset3
152047	1	408094	13	NULL	NULL	0	NULL	1985 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1985 Jordan Husbands ' Fertility Survey ( JHFS ) was designed to assess husbands ' attitudes and behavior toward fertility and family planning .
	manualset3
152048	2	408094	13	NULL	NULL	0	NULL	Jordan Husbands ' Fertility Survey ( JHFS ) 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1985 Jordan Husbands ' Fertility Survey ( JHFS ) was designed to assess husbands ' attitudes and behavior toward fertility and family planning .
	manualset3
152049	3	408094	13	NULL	NULL	0	NULL	husbands	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1985 Jordan Husbands ' Fertility Survey ( JHFS ) was designed to assess husbands ' attitudes and behavior toward fertility and family planning .
	manualset3
152050	4	408094	13	NULL	NULL	0	NULL	attitudes	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1985 Jordan Husbands ' Fertility Survey ( JHFS ) was designed to assess husbands ' attitudes and behavior toward fertility and family planning .
	manualset3
152051	5	408094	13	NULL	NULL	0	NULL	behavior	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1985 Jordan Husbands ' Fertility Survey ( JHFS ) was designed to assess husbands ' attitudes and behavior toward fertility and family planning .
	manualset3
152052	6	408094	13	NULL	NULL	0	NULL	fertility 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1985 Jordan Husbands ' Fertility Survey ( JHFS ) was designed to assess husbands ' attitudes and behavior toward fertility and family planning .
	manualset3
152053	7	408094	13	NULL	NULL	0	NULL	family planning	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1985 Jordan Husbands ' Fertility Survey ( JHFS ) was designed to assess husbands ' attitudes and behavior toward fertility and family planning .
	manualset3
152055	1	408095	13	NULL	NULL	0	NULL	questionnaire	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A questionnaire was designed to assess the amount and type of counseling experiences offered in ESB-accredited communicative disorders programs .
	manualset3
152056	2	408095	13	NULL	NULL	0	NULL	amount 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A questionnaire was designed to assess the amount and type of counseling experiences offered in ESB-accredited communicative disorders programs .
	manualset3
152058	3	408095	13	NULL	NULL	0	NULL	type of counseling experiences	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A questionnaire was designed to assess the amount and type of counseling experiences offered in ESB-accredited communicative disorders programs .
	manualset3
152059	4	408095	13	NULL	NULL	0	NULL	ESB-accredited communicative disorders programs	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A questionnaire was designed to assess the amount and type of counseling experiences offered in ESB-accredited communicative disorders programs .
	manualset3
152061	1	408096	13	NULL	NULL	0	NULL	2 , 886 , 836 bp long genome 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2 , 886 , 836 bp long genome with its four large plasmids of lengths 97 kbp , 132 kbp , 196 kbp and 315 kbp harbors 2 , 741 protein-coding and 58 RNA genes and is a part of the Genomic Encyclopedia of Bacteria and Archaea project .
	manualset3
152062	2	408096	13	NULL	NULL	0	NULL	four large plasmids 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2 , 886 , 836 bp long genome with its four large plasmids of lengths 97 kbp , 132 kbp , 196 kbp and 315 kbp harbors 2 , 741 protein-coding and 58 RNA genes and is a part of the Genomic Encyclopedia of Bacteria and Archaea project .
	manualset3
152063	3	408096	13	NULL	NULL	0	NULL	lengths 97 kbp	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2 , 886 , 836 bp long genome with its four large plasmids of lengths 97 kbp , 132 kbp , 196 kbp and 315 kbp harbors 2 , 741 protein-coding and 58 RNA genes and is a part of the Genomic Encyclopedia of Bacteria and Archaea project .
	manualset3
152064	4	408096	13	NULL	NULL	0	NULL	132 kbp	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2 , 886 , 836 bp long genome with its four large plasmids of lengths 97 kbp , 132 kbp , 196 kbp and 315 kbp harbors 2 , 741 protein-coding and 58 RNA genes and is a part of the Genomic Encyclopedia of Bacteria and Archaea project .
	manualset3
152065	5	408096	13	NULL	NULL	0	NULL	196 kbp	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2 , 886 , 836 bp long genome with its four large plasmids of lengths 97 kbp , 132 kbp , 196 kbp and 315 kbp harbors 2 , 741 protein-coding and 58 RNA genes and is a part of the Genomic Encyclopedia of Bacteria and Archaea project .
	manualset3
152067	6	408096	13	NULL	NULL	0	NULL	15 kbp 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2 , 886 , 836 bp long genome with its four large plasmids of lengths 97 kbp , 132 kbp , 196 kbp and 315 kbp harbors 2 , 741 protein-coding and 58 RNA genes and is a part of the Genomic Encyclopedia of Bacteria and Archaea project .
	manualset3
152068	7	408096	13	NULL	NULL	0	NULL	harbors	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2 , 886 , 836 bp long genome with its four large plasmids of lengths 97 kbp , 132 kbp , 196 kbp and 315 kbp harbors 2 , 741 protein-coding and 58 RNA genes and is a part of the Genomic Encyclopedia of Bacteria and Archaea project .
	manualset3
152069	8	408096	13	NULL	NULL	0	NULL	2 , 741 protein-coding genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2 , 886 , 836 bp long genome with its four large plasmids of lengths 97 kbp , 132 kbp , 196 kbp and 315 kbp harbors 2 , 741 protein-coding and 58 RNA genes and is a part of the Genomic Encyclopedia of Bacteria and Archaea project .
	manualset3
152071	9	408096	13	NULL	NULL	0	NULL	58 RNA genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2 , 886 , 836 bp long genome with its four large plasmids of lengths 97 kbp , 132 kbp , 196 kbp and 315 kbp harbors 2 , 741 protein-coding and 58 RNA genes and is a part of the Genomic Encyclopedia of Bacteria and Archaea project .
	manualset3
152073	10	408096	13	NULL	NULL	0	NULL	Genomic Encyclopedia	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2 , 886 , 836 bp long genome with its four large plasmids of lengths 97 kbp , 132 kbp , 196 kbp and 315 kbp harbors 2 , 741 protein-coding and 58 RNA genes and is a part of the Genomic Encyclopedia of Bacteria and Archaea project .
	manualset3
152074	11	408096	13	NULL	NULL	0	NULL	Bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2 , 886 , 836 bp long genome with its four large plasmids of lengths 97 kbp , 132 kbp , 196 kbp and 315 kbp harbors 2 , 741 protein-coding and 58 RNA genes and is a part of the Genomic Encyclopedia of Bacteria and Archaea project .
	manualset3
152075	12	408096	13	NULL	NULL	0	NULL	Archaea	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2 , 886 , 836 bp long genome with its four large plasmids of lengths 97 kbp , 132 kbp , 196 kbp and 315 kbp harbors 2 , 741 protein-coding and 58 RNA genes and is a part of the Genomic Encyclopedia of Bacteria and Archaea project .
	manualset3
152076	13	408096	13	NULL	NULL	0	NULL	project 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2 , 886 , 836 bp long genome with its four large plasmids of lengths 97 kbp , 132 kbp , 196 kbp and 315 kbp harbors 2 , 741 protein-coding and 58 RNA genes and is a part of the Genomic Encyclopedia of Bacteria and Archaea project .
	manualset3
152077	1	408097	13	NULL	NULL	0	NULL	2-10 day incubation period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2-10 day incubation period meant that cases were dispersed across Pennsylvania at time of onset , and matters were further complicated by the lack of a centralised record of attendance of the convention .
	manualset3
152078	2	408097	13	NULL	NULL	0	NULL	Pennsylvania 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2-10 day incubation period meant that cases were dispersed across Pennsylvania at time of onset , and matters were further complicated by the lack of a centralised record of attendance of the convention .
	manualset3
152079	3	408097	13	NULL	NULL	0	NULL	time of onset 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2-10 day incubation period meant that cases were dispersed across Pennsylvania at time of onset , and matters were further complicated by the lack of a centralised record of attendance of the convention .
	manualset3
152080	4	408097	13	NULL	NULL	0	NULL	matters	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2-10 day incubation period meant that cases were dispersed across Pennsylvania at time of onset , and matters were further complicated by the lack of a centralised record of attendance of the convention .
	manualset3
152081	5	408097	13	NULL	NULL	0	NULL	lack 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2-10 day incubation period meant that cases were dispersed across Pennsylvania at time of onset , and matters were further complicated by the lack of a centralised record of attendance of the convention .
	manualset3
152083	6	408097	13	NULL	NULL	0	NULL	record	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2-10 day incubation period meant that cases were dispersed across Pennsylvania at time of onset , and matters were further complicated by the lack of a centralised record of attendance of the convention .
	manualset3
152084	7	408097	13	NULL	NULL	0	NULL	attendance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2-10 day incubation period meant that cases were dispersed across Pennsylvania at time of onset , and matters were further complicated by the lack of a centralised record of attendance of the convention .
	manualset3
152085	8	408097	13	NULL	NULL	0	NULL	convention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2-10 day incubation period meant that cases were dispersed across Pennsylvania at time of onset , and matters were further complicated by the lack of a centralised record of attendance of the convention .
	manualset3
152088	1	408098	13	NULL	NULL	0	NULL	2 groups	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2 groups were comparable with regard to prognostic factors .
	manualset3
152090	2	408098	13	NULL	NULL	0	NULL	prognostic factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2 groups were comparable with regard to prognostic factors .
	manualset3
152092	1	408099	13	NULL	NULL	0	NULL	 2 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2 patients with complete remission did not show LD ARA-C-induced hypoplasia of bone marrow , although 1 had hypoplastic AML before therapy .
	manualset3
152093	2	408099	13	NULL	NULL	0	NULL	remission	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2 patients with complete remission did not show LD ARA-C-induced hypoplasia of bone marrow , although 1 had hypoplastic AML before therapy .
	manualset3
152094	3	408099	13	NULL	NULL	0	NULL	LD ARA-C-induced hypoplasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2 patients with complete remission did not show LD ARA-C-induced hypoplasia of bone marrow , although 1 had hypoplastic AML before therapy .
	manualset3
152095	4	408099	13	NULL	NULL	0	NULL	bone marrow	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2 patients with complete remission did not show LD ARA-C-induced hypoplasia of bone marrow , although 1 had hypoplastic AML before therapy .
	manualset3
152096	5	408099	13	NULL	NULL	0	NULL	1 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2 patients with complete remission did not show LD ARA-C-induced hypoplasia of bone marrow , although 1 had hypoplastic AML before therapy .
	manualset3
152097	6	408099	13	NULL	NULL	0	NULL	hypoplastic AML 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2 patients with complete remission did not show LD ARA-C-induced hypoplasia of bone marrow , although 1 had hypoplastic AML before therapy .
	manualset3
152099	7	408099	13	NULL	NULL	0	NULL	therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2 patients with complete remission did not show LD ARA-C-induced hypoplasia of bone marrow , although 1 had hypoplastic AML before therapy .
	manualset3
152101	1	408100	13	NULL	NULL	0	NULL	201Tl/99Tcm-MIBI early ratio	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The 201Tl/99Tcm-MIBI early ratio of glioblastoma multiforme was significantly higher than that of metastatic brain tumor .
	manualset3
152103	2	408100	13	NULL	NULL	0	NULL	glioblastoma multiforme 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The 201Tl/99Tcm-MIBI early ratio of glioblastoma multiforme was significantly higher than that of metastatic brain tumor .
	manualset3
152105	3	408100	13	NULL	NULL	0	NULL	metastatic brain tumor 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The 201Tl/99Tcm-MIBI early ratio of glioblastoma multiforme was significantly higher than that of metastatic brain tumor .
	manualset3
152106	1	408101	13	NULL	NULL	0	NULL	 204-kDa smooth muscle myosin heavy chain ( MHC )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The 204-kDa smooth muscle myosin heavy chain ( MHC ) from rat aorta smooth muscle cells was found to be phosphorylated following isolation of myosin from strips of intact aorta as well as from primary cultures of aorta cells .
	manualset3
152107	2	408101	13	NULL	NULL	0	NULL	rat aorta smooth muscle cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The 204-kDa smooth muscle myosin heavy chain ( MHC ) from rat aorta smooth muscle cells was found to be phosphorylated following isolation of myosin from strips of intact aorta as well as from primary cultures of aorta cells .
	manualset3
152108	3	408101	13	NULL	NULL	0	NULL	 isolation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The 204-kDa smooth muscle myosin heavy chain ( MHC ) from rat aorta smooth muscle cells was found to be phosphorylated following isolation of myosin from strips of intact aorta as well as from primary cultures of aorta cells .
	manualset3
152109	4	408101	13	NULL	NULL	0	NULL	myosin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The 204-kDa smooth muscle myosin heavy chain ( MHC ) from rat aorta smooth muscle cells was found to be phosphorylated following isolation of myosin from strips of intact aorta as well as from primary cultures of aorta cells .
	manualset3
152110	5	408101	13	NULL	NULL	0	NULL	strips of intact aorta 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The 204-kDa smooth muscle myosin heavy chain ( MHC ) from rat aorta smooth muscle cells was found to be phosphorylated following isolation of myosin from strips of intact aorta as well as from primary cultures of aorta cells .
	manualset3
152111	6	408101	13	NULL	NULL	0	NULL	primary cultures of aorta cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The 204-kDa smooth muscle myosin heavy chain ( MHC ) from rat aorta smooth muscle cells was found to be phosphorylated following isolation of myosin from strips of intact aorta as well as from primary cultures of aorta cells .
	manualset3
152115	1	408102	13	NULL	NULL	0	NULL	21d_resynch heifers	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The 21d_resynch heifers were diagnosed for pregnancy on d 18 after a TAI ( d 0 ) by using predetermined cut-off values for 2 ' -5 ' oligoadenylate synthetase 1 ( Oas1 ) gene expression in leukocytes and plasma progesterone concentration .
	manualset3
152116	2	408102	13	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The 21d_resynch heifers were diagnosed for pregnancy on d 18 after a TAI ( d 0 ) by using predetermined cut-off values for 2 ' -5 ' oligoadenylate synthetase 1 ( Oas1 ) gene expression in leukocytes and plasma progesterone concentration .
	manualset3
152117	3	408102	13	NULL	NULL	0	NULL	d 18 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The 21d_resynch heifers were diagnosed for pregnancy on d 18 after a TAI ( d 0 ) by using predetermined cut-off values for 2 ' -5 ' oligoadenylate synthetase 1 ( Oas1 ) gene expression in leukocytes and plasma progesterone concentration .
	manualset3
152118	4	408102	13	NULL	NULL	0	NULL	TAI	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The 21d_resynch heifers were diagnosed for pregnancy on d 18 after a TAI ( d 0 ) by using predetermined cut-off values for 2 ' -5 ' oligoadenylate synthetase 1 ( Oas1 ) gene expression in leukocytes and plasma progesterone concentration .
	manualset3
152119	5	408102	13	NULL	NULL	0	NULL	d 0	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The 21d_resynch heifers were diagnosed for pregnancy on d 18 after a TAI ( d 0 ) by using predetermined cut-off values for 2 ' -5 ' oligoadenylate synthetase 1 ( Oas1 ) gene expression in leukocytes and plasma progesterone concentration .
	manualset3
152120	6	408102	13	NULL	NULL	0	NULL	cut-off values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 21d_resynch heifers were diagnosed for pregnancy on d 18 after a TAI ( d 0 ) by using predetermined cut-off values for 2 ' -5 ' oligoadenylate synthetase 1 ( Oas1 ) gene expression in leukocytes and plasma progesterone concentration .
	manualset3
152121	7	408102	13	NULL	NULL	0	NULL	 2 ' -5 ' oligoadenylate synthetase 1 ( Oas1 ) gene expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 21d_resynch heifers were diagnosed for pregnancy on d 18 after a TAI ( d 0 ) by using predetermined cut-off values for 2 ' -5 ' oligoadenylate synthetase 1 ( Oas1 ) gene expression in leukocytes and plasma progesterone concentration .
	manualset3
152122	8	408102	13	NULL	NULL	0	NULL	leukocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The 21d_resynch heifers were diagnosed for pregnancy on d 18 after a TAI ( d 0 ) by using predetermined cut-off values for 2 ' -5 ' oligoadenylate synthetase 1 ( Oas1 ) gene expression in leukocytes and plasma progesterone concentration .
	manualset3
152123	9	408102	13	NULL	NULL	0	NULL	plasma progesterone concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 21d_resynch heifers were diagnosed for pregnancy on d 18 after a TAI ( d 0 ) by using predetermined cut-off values for 2 ' -5 ' oligoadenylate synthetase 1 ( Oas1 ) gene expression in leukocytes and plasma progesterone concentration .
	manualset3
152124	1	408103	13	NULL	NULL	0	NULL	235-1 pituitary tumor clone 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The 235-1 pituitary tumor clone was utilized to study prolactin secretion after perturbing cyclic AMP and calcium metabolism .
	manualset3
152126	2	408103	13	NULL	NULL	0	NULL	prolactin secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 235-1 pituitary tumor clone was utilized to study prolactin secretion after perturbing cyclic AMP and calcium metabolism .
	manualset3
152128	3	408103	13	NULL	NULL	0	NULL	cyclic AMP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The 235-1 pituitary tumor clone was utilized to study prolactin secretion after perturbing cyclic AMP and calcium metabolism .
	manualset3
152129	4	408103	13	NULL	NULL	0	NULL	calcium metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 235-1 pituitary tumor clone was utilized to study prolactin secretion after perturbing cyclic AMP and calcium metabolism .
	manualset3
152130	1	408104	13	NULL	NULL	0	NULL	24-hour	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The 24-hour LABA will likely be combined with a 24-hour anticholinergic to treat chronic obstructive pulmonary disease .
	manualset3
152131	2	408104	13	NULL	NULL	0	NULL	LABA 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The 24-hour LABA will likely be combined with a 24-hour anticholinergic to treat chronic obstructive pulmonary disease .
	manualset3
152132	3	408104	13	NULL	NULL	0	NULL	24-hour	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The 24-hour LABA will likely be combined with a 24-hour anticholinergic to treat chronic obstructive pulmonary disease .
	manualset3
152134	4	408104	13	NULL	NULL	0	NULL	chronic obstructive pulmonary disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The 24-hour LABA will likely be combined with a 24-hour anticholinergic to treat chronic obstructive pulmonary disease .
	manualset3
152136	1	408105	13	NULL	NULL	0	NULL	questionnaire 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A questionnaire was presented to 3 , 450 workers who had exposure to dust during the course of flour milling ( 528 ) , bread baking ( 1 , 756 ) , cake baking ( 209 ) and other activities in food preparation ( 957 ) .
	manualset3
152137	2	408105	13	NULL	NULL	0	NULL	 3 , 450 workers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A questionnaire was presented to 3 , 450 workers who had exposure to dust during the course of flour milling ( 528 ) , bread baking ( 1 , 756 ) , cake baking ( 209 ) and other activities in food preparation ( 957 ) .
	manualset3
152138	3	408105	13	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A questionnaire was presented to 3 , 450 workers who had exposure to dust during the course of flour milling ( 528 ) , bread baking ( 1 , 756 ) , cake baking ( 209 ) and other activities in food preparation ( 957 ) .
	manualset3
152139	4	408105	13	NULL	NULL	0	NULL	course of flour milling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A questionnaire was presented to 3 , 450 workers who had exposure to dust during the course of flour milling ( 528 ) , bread baking ( 1 , 756 ) , cake baking ( 209 ) and other activities in food preparation ( 957 ) .
	manualset3
152140	5	408105	13	NULL	NULL	0	NULL	528	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A questionnaire was presented to 3 , 450 workers who had exposure to dust during the course of flour milling ( 528 ) , bread baking ( 1 , 756 ) , cake baking ( 209 ) and other activities in food preparation ( 957 ) .
	manualset3
152141	6	408105	13	NULL	NULL	0	NULL	bread baking	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A questionnaire was presented to 3 , 450 workers who had exposure to dust during the course of flour milling ( 528 ) , bread baking ( 1 , 756 ) , cake baking ( 209 ) and other activities in food preparation ( 957 ) .
	manualset3
152142	7	408105	13	NULL	NULL	0	NULL	1 , 756 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A questionnaire was presented to 3 , 450 workers who had exposure to dust during the course of flour milling ( 528 ) , bread baking ( 1 , 756 ) , cake baking ( 209 ) and other activities in food preparation ( 957 ) .
	manualset3
152143	8	408105	13	NULL	NULL	0	NULL	cake baking	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A questionnaire was presented to 3 , 450 workers who had exposure to dust during the course of flour milling ( 528 ) , bread baking ( 1 , 756 ) , cake baking ( 209 ) and other activities in food preparation ( 957 ) .
	manualset3
152144	9	408105	13	NULL	NULL	0	NULL	209 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A questionnaire was presented to 3 , 450 workers who had exposure to dust during the course of flour milling ( 528 ) , bread baking ( 1 , 756 ) , cake baking ( 209 ) and other activities in food preparation ( 957 ) .
	manualset3
152146	10	408105	13	NULL	NULL	0	NULL	activities 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A questionnaire was presented to 3 , 450 workers who had exposure to dust during the course of flour milling ( 528 ) , bread baking ( 1 , 756 ) , cake baking ( 209 ) and other activities in food preparation ( 957 ) .
	manualset3
152147	11	408105	13	NULL	NULL	0	NULL	food preparation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A questionnaire was presented to 3 , 450 workers who had exposure to dust during the course of flour milling ( 528 ) , bread baking ( 1 , 756 ) , cake baking ( 209 ) and other activities in food preparation ( 957 ) .
	manualset3
152148	12	408105	13	NULL	NULL	0	NULL	957 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A questionnaire was presented to 3 , 450 workers who had exposure to dust during the course of flour milling ( 528 ) , bread baking ( 1 , 756 ) , cake baking ( 209 ) and other activities in food preparation ( 957 ) .
	manualset3
152149	1	408106	13	NULL	NULL	0	NULL	 24-hour 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The 24-hour intakes of several key macronutrients and micronutrients also improved .
	manualset3
152150	2	408106	13	NULL	NULL	0	NULL	 intakes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 24-hour intakes of several key macronutrients and micronutrients also improved .
	manualset3
152151	3	408106	13	NULL	NULL	0	NULL	key macronutrients 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The 24-hour intakes of several key macronutrients and micronutrients also improved .
	manualset3
152152	4	408106	13	NULL	NULL	0	NULL	micronutrients	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The 24-hour intakes of several key macronutrients and micronutrients also improved .
	manualset3
152154	1	408107	13	NULL	NULL	0	NULL	24-wk	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The 24-wk intervention included a lipid-based nutrient supplement , education , promotion of existing clinical services , and social support .
	manualset3
152155	2	408107	13	NULL	NULL	0	NULL	intervention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 24-wk intervention included a lipid-based nutrient supplement , education , promotion of existing clinical services , and social support .
	manualset3
152156	3	408107	13	NULL	NULL	0	NULL	 lipid-based nutrient supplement 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The 24-wk intervention included a lipid-based nutrient supplement , education , promotion of existing clinical services , and social support .
	manualset3
152157	4	408107	13	NULL	NULL	0	NULL	education	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 24-wk intervention included a lipid-based nutrient supplement , education , promotion of existing clinical services , and social support .
	manualset3
152158	5	408107	13	NULL	NULL	0	NULL	promotion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 24-wk intervention included a lipid-based nutrient supplement , education , promotion of existing clinical services , and social support .
	manualset3
152160	6	408107	13	NULL	NULL	0	NULL	clinical services 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The 24-wk intervention included a lipid-based nutrient supplement , education , promotion of existing clinical services , and social support .
	manualset3
152161	7	408107	13	NULL	NULL	0	NULL	social support	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 24-wk intervention included a lipid-based nutrient supplement , education , promotion of existing clinical services , and social support .
	manualset3
152164	1	408108	13	NULL	NULL	0	NULL	29th session	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 29th session of the UN Commission on Population and Development ( February 26 to March 1 , 1996 ) focused on reproductive health and rights , including population IEC ( information , education , and communication ) .
	manualset3
152165	2	408108	13	NULL	NULL	0	NULL	UN Commission	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 29th session of the UN Commission on Population and Development ( February 26 to March 1 , 1996 ) focused on reproductive health and rights , including population IEC ( information , education , and communication ) .
	manualset3
152166	3	408108	13	NULL	NULL	0	NULL	Population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The 29th session of the UN Commission on Population and Development ( February 26 to March 1 , 1996 ) focused on reproductive health and rights , including population IEC ( information , education , and communication ) .
	manualset3
152167	4	408108	13	NULL	NULL	0	NULL	Development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 29th session of the UN Commission on Population and Development ( February 26 to March 1 , 1996 ) focused on reproductive health and rights , including population IEC ( information , education , and communication ) .
	manualset3
152168	5	408108	13	NULL	NULL	0	NULL	February 26 to March 1 , 1996	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The 29th session of the UN Commission on Population and Development ( February 26 to March 1 , 1996 ) focused on reproductive health and rights , including population IEC ( information , education , and communication ) .
	manualset3
152169	6	408108	13	NULL	NULL	0	NULL	reproductive health 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The 29th session of the UN Commission on Population and Development ( February 26 to March 1 , 1996 ) focused on reproductive health and rights , including population IEC ( information , education , and communication ) .
	manualset3
152170	7	408108	13	NULL	NULL	0	NULL	rights	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 29th session of the UN Commission on Population and Development ( February 26 to March 1 , 1996 ) focused on reproductive health and rights , including population IEC ( information , education , and communication ) .
	manualset3
152171	8	408108	13	NULL	NULL	0	NULL	population IEC	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 29th session of the UN Commission on Population and Development ( February 26 to March 1 , 1996 ) focused on reproductive health and rights , including population IEC ( information , education , and communication ) .
	manualset3
152172	9	408108	13	NULL	NULL	0	NULL	information	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 29th session of the UN Commission on Population and Development ( February 26 to March 1 , 1996 ) focused on reproductive health and rights , including population IEC ( information , education , and communication ) .
	manualset3
152173	10	408108	13	NULL	NULL	0	NULL	education	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 29th session of the UN Commission on Population and Development ( February 26 to March 1 , 1996 ) focused on reproductive health and rights , including population IEC ( information , education , and communication ) .
	manualset3
152174	11	408108	13	NULL	NULL	0	NULL	communication 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 29th session of the UN Commission on Population and Development ( February 26 to March 1 , 1996 ) focused on reproductive health and rights , including population IEC ( information , education , and communication ) .
	manualset3
152175	1	408109	13	NULL	NULL	0	NULL	300-kDa precursor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The 300-kDa precursor was converted into mature mucin after extensive glycosylation and sulfation .
	manualset3
152176	2	408109	13	NULL	NULL	0	NULL	mature mucin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The 300-kDa precursor was converted into mature mucin after extensive glycosylation and sulfation .
	manualset3
152177	3	408109	13	NULL	NULL	0	NULL	glycosylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 300-kDa precursor was converted into mature mucin after extensive glycosylation and sulfation .
	manualset3
152179	4	408109	13	NULL	NULL	0	NULL	sulfation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 300-kDa precursor was converted into mature mucin after extensive glycosylation and sulfation .
	manualset3
152180	1	408110	13	NULL	NULL	0	NULL	3D-conformal treatment planning	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The 3D-conformal treatment planning optimizes dose distribution to the whole breast and to the tumor bed and lessens the normal tissue irradiation ( heart and ipsilateral lung ) .
	manualset3
152181	2	408110	13	NULL	NULL	0	NULL	dose distribution 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The 3D-conformal treatment planning optimizes dose distribution to the whole breast and to the tumor bed and lessens the normal tissue irradiation ( heart and ipsilateral lung ) .
	manualset3
152182	3	408110	13	NULL	NULL	0	NULL	breast 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The 3D-conformal treatment planning optimizes dose distribution to the whole breast and to the tumor bed and lessens the normal tissue irradiation ( heart and ipsilateral lung ) .
	manualset3
152183	4	408110	13	NULL	NULL	0	NULL	tumor bed	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The 3D-conformal treatment planning optimizes dose distribution to the whole breast and to the tumor bed and lessens the normal tissue irradiation ( heart and ipsilateral lung ) .
	manualset3
152185	5	408110	13	NULL	NULL	0	NULL	normal tissue irradiation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The 3D-conformal treatment planning optimizes dose distribution to the whole breast and to the tumor bed and lessens the normal tissue irradiation ( heart and ipsilateral lung ) .
	manualset3
152186	6	408110	13	NULL	NULL	0	NULL	heart 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The 3D-conformal treatment planning optimizes dose distribution to the whole breast and to the tumor bed and lessens the normal tissue irradiation ( heart and ipsilateral lung ) .
	manualset3
152187	7	408110	13	NULL	NULL	0	NULL	ipsilateral lung	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The 3D-conformal treatment planning optimizes dose distribution to the whole breast and to the tumor bed and lessens the normal tissue irradiation ( heart and ipsilateral lung ) .
	manualset3
152236	1	408111	13	NULL	NULL	0	NULL	rare type of EnS 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A quite rare type of EnS - motile bacteria - was found in ciliates of the same two classes as well , either in the cytoplasm ( Heterotrichea ) or in the macronucleus and its perinuclear space ( Oligohymenophorea ) .
	manualset3
152237	2	408111	13	NULL	NULL	0	NULL	motile bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A quite rare type of EnS - motile bacteria - was found in ciliates of the same two classes as well , either in the cytoplasm ( Heterotrichea ) or in the macronucleus and its perinuclear space ( Oligohymenophorea ) .
	manualset3
152238	3	408111	13	NULL	NULL	0	NULL	ciliates 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A quite rare type of EnS - motile bacteria - was found in ciliates of the same two classes as well , either in the cytoplasm ( Heterotrichea ) or in the macronucleus and its perinuclear space ( Oligohymenophorea ) .
	manualset3
152239	4	408111	13	NULL	NULL	0	NULL	two classes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A quite rare type of EnS - motile bacteria - was found in ciliates of the same two classes as well , either in the cytoplasm ( Heterotrichea ) or in the macronucleus and its perinuclear space ( Oligohymenophorea ) .
	manualset3
152240	5	408111	13	NULL	NULL	0	NULL	cytoplasm	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A quite rare type of EnS - motile bacteria - was found in ciliates of the same two classes as well , either in the cytoplasm ( Heterotrichea ) or in the macronucleus and its perinuclear space ( Oligohymenophorea ) .
	manualset3
152241	6	408111	13	NULL	NULL	0	NULL	Heterotrichea	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A quite rare type of EnS - motile bacteria - was found in ciliates of the same two classes as well , either in the cytoplasm ( Heterotrichea ) or in the macronucleus and its perinuclear space ( Oligohymenophorea ) .
	manualset3
152242	7	408111	13	NULL	NULL	0	NULL	macronucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A quite rare type of EnS - motile bacteria - was found in ciliates of the same two classes as well , either in the cytoplasm ( Heterotrichea ) or in the macronucleus and its perinuclear space ( Oligohymenophorea ) .
	manualset3
152243	8	408111	13	NULL	NULL	0	NULL	perinuclear space 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A quite rare type of EnS - motile bacteria - was found in ciliates of the same two classes as well , either in the cytoplasm ( Heterotrichea ) or in the macronucleus and its perinuclear space ( Oligohymenophorea ) .
	manualset3
152244	9	408111	13	NULL	NULL	0	NULL	Oligohymenophorea	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A quite rare type of EnS - motile bacteria - was found in ciliates of the same two classes as well , either in the cytoplasm ( Heterotrichea ) or in the macronucleus and its perinuclear space ( Oligohymenophorea ) .
	manualset3
152245	1	408112	13	NULL	NULL	0	NULL	4-Cl benzoyl derivative	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The 4-Cl benzoyl derivative , compound 29u , was the most active one with IC ( 50 ) values in the range 0.049-2 .6 M .
	manualset3
152246	2	408112	13	NULL	NULL	0	NULL	compound 29u	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The 4-Cl benzoyl derivative , compound 29u , was the most active one with IC ( 50 ) values in the range 0.049-2 .6 M .
	manualset3
152247	3	408112	13	NULL	NULL	0	NULL	IC ( 50 ) values	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 4-Cl benzoyl derivative , compound 29u , was the most active one with IC ( 50 ) values in the range 0.049-2 .6 M .
	manualset3
152248	4	408112	13	NULL	NULL	0	NULL	range 0.049-2 .6 M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 4-Cl benzoyl derivative , compound 29u , was the most active one with IC ( 50 ) values in the range 0.049-2 .6 M .
	manualset3
152249	1	408113	13	NULL	NULL	0	NULL	 4-km	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 4-km modeling configuration is also recommended for the development of air pollution control strategies .
	manualset3
152250	2	408113	13	NULL	NULL	0	NULL	modeling configuration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 4-km modeling configuration is also recommended for the development of air pollution control strategies .
	manualset3
152251	3	408113	13	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 4-km modeling configuration is also recommended for the development of air pollution control strategies .
	manualset3
152252	4	408113	13	NULL	NULL	0	NULL	air pollution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 4-km modeling configuration is also recommended for the development of air pollution control strategies .
	manualset3
152253	5	408113	13	NULL	NULL	0	NULL	control strategies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 4-km modeling configuration is also recommended for the development of air pollution control strategies .
	manualset3
152254	1	408114	13	NULL	NULL	0	NULL	40-fluted finishing burs 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The 40-fluted and 12-fluted finishing burs ranked second and third , respectively , and the superfine diamond stone was judged to produce the roughest and least distinct bevel .
	manualset3
152255	2	408114	13	NULL	NULL	0	NULL	12-fluted finishing burs 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The 40-fluted and 12-fluted finishing burs ranked second and third , respectively , and the superfine diamond stone was judged to produce the roughest and least distinct bevel .
	manualset3
152256	3	408114	13	NULL	NULL	0	NULL	second 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 40-fluted and 12-fluted finishing burs ranked second and third , respectively , and the superfine diamond stone was judged to produce the roughest and least distinct bevel .
	manualset3
152257	4	408114	13	NULL	NULL	0	NULL	third	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 40-fluted and 12-fluted finishing burs ranked second and third , respectively , and the superfine diamond stone was judged to produce the roughest and least distinct bevel .
	manualset3
152258	5	408114	13	NULL	NULL	0	NULL	superfine diamond stone 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The 40-fluted and 12-fluted finishing burs ranked second and third , respectively , and the superfine diamond stone was judged to produce the roughest and least distinct bevel .
	manualset3
152259	1	408115	13	NULL	NULL	0	NULL	434 ( G ) C ) polymorphism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 434 ( G ) C ) polymorphism within the coding sequence of Eosinophil Cationic Protein ( ECP ) correlates with the natural course of Schistosoma mansoni infection .
	manualset3
152260	2	408115	13	NULL	NULL	0	NULL	coding sequence 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The 434 ( G ) C ) polymorphism within the coding sequence of Eosinophil Cationic Protein ( ECP ) correlates with the natural course of Schistosoma mansoni infection .
	manualset3
152261	3	408115	13	NULL	NULL	0	NULL	Eosinophil Cationic Protein ( ECP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The 434 ( G ) C ) polymorphism within the coding sequence of Eosinophil Cationic Protein ( ECP ) correlates with the natural course of Schistosoma mansoni infection .
	manualset3
152262	4	408115	13	NULL	NULL	0	NULL	natural course	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The 434 ( G ) C ) polymorphism within the coding sequence of Eosinophil Cationic Protein ( ECP ) correlates with the natural course of Schistosoma mansoni infection .
	manualset3
152263	5	408115	13	NULL	NULL	0	NULL	Schistosoma mansoni infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The 434 ( G ) C ) polymorphism within the coding sequence of Eosinophil Cationic Protein ( ECP ) correlates with the natural course of Schistosoma mansoni infection .
	manualset3
152264	1	408116	13	NULL	NULL	0	NULL	45Ca2 + uptake 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 45Ca2 + uptake by the transformed cells was increased as compared to normal cells .
	manualset3
152265	2	408116	13	NULL	NULL	0	NULL	transformed cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The 45Ca2 + uptake by the transformed cells was increased as compared to normal cells .
	manualset3
152266	3	408116	13	NULL	NULL	0	NULL	normal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The 45Ca2 + uptake by the transformed cells was increased as compared to normal cells .
	manualset3
152267	1	408117	13	NULL	NULL	0	NULL	4S TMV capsid protein monomers 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The 4S TMV capsid protein monomers were isolated from TMV particles purified from infected plants of Nicotiana tabacum L. and were induced to form 20S stacked disc aggregates .
	manualset3
152268	2	408117	13	NULL	NULL	0	NULL	TMV particles	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The 4S TMV capsid protein monomers were isolated from TMV particles purified from infected plants of Nicotiana tabacum L. and were induced to form 20S stacked disc aggregates .
	manualset3
152269	3	408117	13	NULL	NULL	0	NULL	plants of Nicotiana tabacum L.	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The 4S TMV capsid protein monomers were isolated from TMV particles purified from infected plants of Nicotiana tabacum L. and were induced to form 20S stacked disc aggregates .
	manualset3
152270	4	408117	13	NULL	NULL	0	NULL	20S stacked disc aggregates	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 4S TMV capsid protein monomers were isolated from TMV particles purified from infected plants of Nicotiana tabacum L. and were induced to form 20S stacked disc aggregates .
	manualset3
152271	1	408118	13	NULL	NULL	0	NULL	Characteristic changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Characteristic changes in the pattern of distribution of muscarinic receptors in the exstrophic bladder wall ) .
	manualset3
152272	2	408118	13	NULL	NULL	0	NULL	 pattern 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Characteristic changes in the pattern of distribution of muscarinic receptors in the exstrophic bladder wall ) .
	manualset3
152273	3	408118	13	NULL	NULL	0	NULL	distribution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Characteristic changes in the pattern of distribution of muscarinic receptors in the exstrophic bladder wall ) .
	manualset3
152274	4	408118	13	NULL	NULL	0	NULL	muscarinic receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Characteristic changes in the pattern of distribution of muscarinic receptors in the exstrophic bladder wall ) .
	manualset3
152275	5	408118	13	NULL	NULL	0	NULL	exstrophic bladder wall 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Characteristic changes in the pattern of distribution of muscarinic receptors in the exstrophic bladder wall ) .
	manualset3
152276	1	408119	13	NULL	NULL	0	NULL	rabbit antiserum ( R917 ) 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A rabbit antiserum ( R917 ) was raised to a purified fraction of bovine brain basic fibroblast growth factor ( bFGF ) .
	manualset3
152277	2	408119	13	NULL	NULL	0	NULL	purified fraction	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A rabbit antiserum ( R917 ) was raised to a purified fraction of bovine brain basic fibroblast growth factor ( bFGF ) .
	manualset3
152278	3	408119	13	NULL	NULL	0	NULL	bovine brain basic fibroblast growth factor ( bFGF )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A rabbit antiserum ( R917 ) was raised to a purified fraction of bovine brain basic fibroblast growth factor ( bFGF ) .
	manualset3
152279	1	408120	13	NULL	NULL	0	NULL	5-hydroxytryptamine ( 5-HT , serotonin ) system	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 5-hydroxytryptamine ( 5-HT , serotonin ) system has been implicated in the pathophysiology and treatment of schizophrenia .
	manualset3
152280	2	408120	13	NULL	NULL	0	NULL	pathophysiology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The 5-hydroxytryptamine ( 5-HT , serotonin ) system has been implicated in the pathophysiology and treatment of schizophrenia .
	manualset3
152281	3	408120	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The 5-hydroxytryptamine ( 5-HT , serotonin ) system has been implicated in the pathophysiology and treatment of schizophrenia .
	manualset3
152282	4	408120	13	NULL	NULL	0	NULL	schizophrenia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The 5-hydroxytryptamine ( 5-HT , serotonin ) system has been implicated in the pathophysiology and treatment of schizophrenia .
	manualset3
152283	1	408121	13	NULL	NULL	0	NULL	5-year	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The 5-year relapse-free survival for primary vaginal carcinoma was 88 % for Stage I , 44 % for Stage II , 35 % for Stage III , and 0 % for Stage IV .
	manualset3
152284	2	408121	13	NULL	NULL	0	NULL	relapse-free survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The 5-year relapse-free survival for primary vaginal carcinoma was 88 % for Stage I , 44 % for Stage II , 35 % for Stage III , and 0 % for Stage IV .
	manualset3
152285	3	408121	13	NULL	NULL	0	NULL	primary vaginal carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The 5-year relapse-free survival for primary vaginal carcinoma was 88 % for Stage I , 44 % for Stage II , 35 % for Stage III , and 0 % for Stage IV .
	manualset3
152286	4	408121	13	NULL	NULL	0	NULL	 88 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 5-year relapse-free survival for primary vaginal carcinoma was 88 % for Stage I , 44 % for Stage II , 35 % for Stage III , and 0 % for Stage IV .
	manualset3
152287	5	408121	13	NULL	NULL	0	NULL	Stage I 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The 5-year relapse-free survival for primary vaginal carcinoma was 88 % for Stage I , 44 % for Stage II , 35 % for Stage III , and 0 % for Stage IV .
	manualset3
152288	6	408121	13	NULL	NULL	0	NULL	44 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 5-year relapse-free survival for primary vaginal carcinoma was 88 % for Stage I , 44 % for Stage II , 35 % for Stage III , and 0 % for Stage IV .
	manualset3
152289	7	408121	13	NULL	NULL	0	NULL	Stage II	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The 5-year relapse-free survival for primary vaginal carcinoma was 88 % for Stage I , 44 % for Stage II , 35 % for Stage III , and 0 % for Stage IV .
	manualset3
152290	8	408121	13	NULL	NULL	0	NULL	35 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 5-year relapse-free survival for primary vaginal carcinoma was 88 % for Stage I , 44 % for Stage II , 35 % for Stage III , and 0 % for Stage IV .
	manualset3
152291	9	408121	13	NULL	NULL	0	NULL	Stage III 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The 5-year relapse-free survival for primary vaginal carcinoma was 88 % for Stage I , 44 % for Stage II , 35 % for Stage III , and 0 % for Stage IV .
	manualset3
152292	10	408121	13	NULL	NULL	0	NULL	0 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 5-year relapse-free survival for primary vaginal carcinoma was 88 % for Stage I , 44 % for Stage II , 35 % for Stage III , and 0 % for Stage IV .
	manualset3
152293	11	408121	13	NULL	NULL	0	NULL	Stage IV	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The 5-year relapse-free survival for primary vaginal carcinoma was 88 % for Stage I , 44 % for Stage II , 35 % for Stage III , and 0 % for Stage IV .
	manualset3
152294	1	408122	13	NULL	NULL	0	NULL	 5 ' end of the RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The 5 ' end of the RNA in the U2 snRNP is more exposed for reaction with RNase H and with chemical probes when the U2 snRNP is in the 17S form than when it is in the 12S form .
	manualset3
152295	2	408122	13	NULL	NULL	0	NULL	 U2 snRNP	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The 5 ' end of the RNA in the U2 snRNP is more exposed for reaction with RNase H and with chemical probes when the U2 snRNP is in the 17S form than when it is in the 12S form .
	manualset3
152296	3	408122	13	NULL	NULL	0	NULL	reaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 5 ' end of the RNA in the U2 snRNP is more exposed for reaction with RNase H and with chemical probes when the U2 snRNP is in the 17S form than when it is in the 12S form .
	manualset3
152297	4	408122	13	NULL	NULL	0	NULL	RNase H 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The 5 ' end of the RNA in the U2 snRNP is more exposed for reaction with RNase H and with chemical probes when the U2 snRNP is in the 17S form than when it is in the 12S form .
	manualset3
152298	5	408122	13	NULL	NULL	0	NULL	chemical probes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The 5 ' end of the RNA in the U2 snRNP is more exposed for reaction with RNase H and with chemical probes when the U2 snRNP is in the 17S form than when it is in the 12S form .
	manualset3
152299	6	408122	13	NULL	NULL	0	NULL	U2 snRNP	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The 5 ' end of the RNA in the U2 snRNP is more exposed for reaction with RNase H and with chemical probes when the U2 snRNP is in the 17S form than when it is in the 12S form .
	manualset3
152300	7	408122	13	NULL	NULL	0	NULL	17S form 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The 5 ' end of the RNA in the U2 snRNP is more exposed for reaction with RNase H and with chemical probes when the U2 snRNP is in the 17S form than when it is in the 12S form .
	manualset3
152301	8	408122	13	NULL	NULL	0	NULL	12S form	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The 5 ' end of the RNA in the U2 snRNP is more exposed for reaction with RNase H and with chemical probes when the U2 snRNP is in the 17S form than when it is in the 12S form .
	manualset3
152302	1	408123	13	NULL	NULL	0	NULL	50 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 50 % inhibitory doses of erythromycin for the inhibition of translation and 50S subunit assembly in Staphylococcus aureus cells were measured and were found to be identical .
	manualset3
152303	2	408123	13	NULL	NULL	0	NULL	inhibitory doses	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 50 % inhibitory doses of erythromycin for the inhibition of translation and 50S subunit assembly in Staphylococcus aureus cells were measured and were found to be identical .
	manualset3
152304	3	408123	13	NULL	NULL	0	NULL	erythromycin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The 50 % inhibitory doses of erythromycin for the inhibition of translation and 50S subunit assembly in Staphylococcus aureus cells were measured and were found to be identical .
	manualset3
152305	4	408123	13	NULL	NULL	0	NULL	inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 50 % inhibitory doses of erythromycin for the inhibition of translation and 50S subunit assembly in Staphylococcus aureus cells were measured and were found to be identical .
	manualset3
152306	5	408123	13	NULL	NULL	0	NULL	translation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 50 % inhibitory doses of erythromycin for the inhibition of translation and 50S subunit assembly in Staphylococcus aureus cells were measured and were found to be identical .
	manualset3
152307	6	408123	13	NULL	NULL	0	NULL	50S subunit assembly	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 50 % inhibitory doses of erythromycin for the inhibition of translation and 50S subunit assembly in Staphylococcus aureus cells were measured and were found to be identical .
	manualset3
152308	7	408123	13	NULL	NULL	0	NULL	Staphylococcus aureus cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The 50 % inhibitory doses of erythromycin for the inhibition of translation and 50S subunit assembly in Staphylococcus aureus cells were measured and were found to be identical .
	manualset3
152309	1	408124	13	NULL	NULL	0	NULL	50th percentile	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 50th percentile for MAMC in Chinese of both sexes fell below the 25th percentile of the Western population of the same age and sex groups ; ( 3 . )
	manualset3
152310	2	408124	13	NULL	NULL	0	NULL	MAMC	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The 50th percentile for MAMC in Chinese of both sexes fell below the 25th percentile of the Western population of the same age and sex groups ; ( 3 . )
	manualset3
152311	3	408124	13	NULL	NULL	0	NULL	Chinese	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The 50th percentile for MAMC in Chinese of both sexes fell below the 25th percentile of the Western population of the same age and sex groups ; ( 3 . )
	manualset3
152312	4	408124	13	NULL	NULL	0	NULL	sexes	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The 50th percentile for MAMC in Chinese of both sexes fell below the 25th percentile of the Western population of the same age and sex groups ; ( 3 . )
	manualset3
152313	5	408124	13	NULL	NULL	0	NULL	25th percentile	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 50th percentile for MAMC in Chinese of both sexes fell below the 25th percentile of the Western population of the same age and sex groups ; ( 3 . )
	manualset3
152314	6	408124	13	NULL	NULL	0	NULL	Western population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The 50th percentile for MAMC in Chinese of both sexes fell below the 25th percentile of the Western population of the same age and sex groups ; ( 3 . )
	manualset3
152315	7	408124	13	NULL	NULL	0	NULL	age	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 50th percentile for MAMC in Chinese of both sexes fell below the 25th percentile of the Western population of the same age and sex groups ; ( 3 . )
	manualset3
152316	8	408124	13	NULL	NULL	0	NULL	sex groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The 50th percentile for MAMC in Chinese of both sexes fell below the 25th percentile of the Western population of the same age and sex groups ; ( 3 . )
	manualset3
152317	1	408125	13	NULL	NULL	0	NULL	51Cr-ethylenediaminetetraacetic acid ( EDTA ) absorption test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The 51Cr-ethylenediaminetetraacetic acid ( EDTA ) absorption test was evaluated in 83 healthy , male volunteers .
	manualset3
152318	2	408125	13	NULL	NULL	0	NULL	83 healthy , male volunteers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The 51Cr-ethylenediaminetetraacetic acid ( EDTA ) absorption test was evaluated in 83 healthy , male volunteers .
	manualset3
152319	1	408126	13	NULL	NULL	0	NULL	70-kDa fragment	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The 70-kDa fragment binds to gelatin , to fibrin ( with unusually high apparent affinity ) , to heparin ( at low ionic strength ) , and to fixed Staphylococcus aureus cells ; it also contains an acceptor site for factor XIIIa ( plasma transglutaminase ) .
	manualset3
152320	2	408126	13	NULL	NULL	0	NULL	gelatin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The 70-kDa fragment binds to gelatin , to fibrin ( with unusually high apparent affinity ) , to heparin ( at low ionic strength ) , and to fixed Staphylococcus aureus cells ; it also contains an acceptor site for factor XIIIa ( plasma transglutaminase ) .
	manualset3
152321	3	408126	13	NULL	NULL	0	NULL	fibrin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The 70-kDa fragment binds to gelatin , to fibrin ( with unusually high apparent affinity ) , to heparin ( at low ionic strength ) , and to fixed Staphylococcus aureus cells ; it also contains an acceptor site for factor XIIIa ( plasma transglutaminase ) .
	manualset3
152322	4	408126	13	NULL	NULL	0	NULL	apparent affinity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 70-kDa fragment binds to gelatin , to fibrin ( with unusually high apparent affinity ) , to heparin ( at low ionic strength ) , and to fixed Staphylococcus aureus cells ; it also contains an acceptor site for factor XIIIa ( plasma transglutaminase ) .
	manualset3
152323	5	408126	13	NULL	NULL	0	NULL	heparin 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The 70-kDa fragment binds to gelatin , to fibrin ( with unusually high apparent affinity ) , to heparin ( at low ionic strength ) , and to fixed Staphylococcus aureus cells ; it also contains an acceptor site for factor XIIIa ( plasma transglutaminase ) .
	manualset3
152324	6	408126	13	NULL	NULL	0	NULL	low ionic strength	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 70-kDa fragment binds to gelatin , to fibrin ( with unusually high apparent affinity ) , to heparin ( at low ionic strength ) , and to fixed Staphylococcus aureus cells ; it also contains an acceptor site for factor XIIIa ( plasma transglutaminase ) .
	manualset3
152325	7	408126	13	NULL	NULL	0	NULL	Staphylococcus aureus cells	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The 70-kDa fragment binds to gelatin , to fibrin ( with unusually high apparent affinity ) , to heparin ( at low ionic strength ) , and to fixed Staphylococcus aureus cells ; it also contains an acceptor site for factor XIIIa ( plasma transglutaminase ) .
	manualset3
152326	8	408126	13	NULL	NULL	0	NULL	acceptor site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The 70-kDa fragment binds to gelatin , to fibrin ( with unusually high apparent affinity ) , to heparin ( at low ionic strength ) , and to fixed Staphylococcus aureus cells ; it also contains an acceptor site for factor XIIIa ( plasma transglutaminase ) .
	manualset3
152327	9	408126	13	NULL	NULL	0	NULL	factor XIIIa	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The 70-kDa fragment binds to gelatin , to fibrin ( with unusually high apparent affinity ) , to heparin ( at low ionic strength ) , and to fixed Staphylococcus aureus cells ; it also contains an acceptor site for factor XIIIa ( plasma transglutaminase ) .
	manualset3
152328	10	408126	13	NULL	NULL	0	NULL	plasma transglutaminase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The 70-kDa fragment binds to gelatin , to fibrin ( with unusually high apparent affinity ) , to heparin ( at low ionic strength ) , and to fixed Staphylococcus aureus cells ; it also contains an acceptor site for factor XIIIa ( plasma transglutaminase ) .
	manualset3
152329	1	408127	13	NULL	NULL	0	NULL	80-kDa protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The 80-kDa protein is selectively expressed in hemangioblastoma , a tumor characterized by overexpression of GLUT1 .
	manualset3
152330	2	408127	13	NULL	NULL	0	NULL	hemangioblastoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The 80-kDa protein is selectively expressed in hemangioblastoma , a tumor characterized by overexpression of GLUT1 .
	manualset3
152331	3	408127	13	NULL	NULL	0	NULL	tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The 80-kDa protein is selectively expressed in hemangioblastoma , a tumor characterized by overexpression of GLUT1 .
	manualset3
152332	4	408127	13	NULL	NULL	0	NULL	overexpression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 80-kDa protein is selectively expressed in hemangioblastoma , a tumor characterized by overexpression of GLUT1 .
	manualset3
152333	5	408127	13	NULL	NULL	0	NULL	GLUT1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The 80-kDa protein is selectively expressed in hemangioblastoma , a tumor characterized by overexpression of GLUT1 .
	manualset3
152334	1	408128	13	NULL	NULL	0	NULL	86-kDa immediate-early 2 ( IE2 ) protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The 86-kDa immediate-early 2 ( IE2 ) protein of human cytomegalovirus ( HCMV ) is a promiscuous transactivator essential for viral gene expression .
	manualset3
152335	2	408128	13	NULL	NULL	0	NULL	human cytomegalovirus ( HCMV ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The 86-kDa immediate-early 2 ( IE2 ) protein of human cytomegalovirus ( HCMV ) is a promiscuous transactivator essential for viral gene expression .
	manualset3
152336	3	408128	13	NULL	NULL	0	NULL	transactivator 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The 86-kDa immediate-early 2 ( IE2 ) protein of human cytomegalovirus ( HCMV ) is a promiscuous transactivator essential for viral gene expression .
	manualset3
152337	4	408128	13	NULL	NULL	0	NULL	viral gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 86-kDa immediate-early 2 ( IE2 ) protein of human cytomegalovirus ( HCMV ) is a promiscuous transactivator essential for viral gene expression .
	manualset3
152338	1	408129	13	NULL	NULL	0	NULL	90 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 90 % confidence intervals of the ratios of means C ( max ) , AUC ( 0-t ) , AUC ( 0-infinity ) and T ( 1/2 ) all fell within the acceptance range of 0.8-1 .25 , demonstrating the bioequivalence of the two formulations .
	manualset3
152339	2	408129	13	NULL	NULL	0	NULL	confidence intervals	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 90 % confidence intervals of the ratios of means C ( max ) , AUC ( 0-t ) , AUC ( 0-infinity ) and T ( 1/2 ) all fell within the acceptance range of 0.8-1 .25 , demonstrating the bioequivalence of the two formulations .
	manualset3
152340	3	408129	13	NULL	NULL	0	NULL	ratios	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 90 % confidence intervals of the ratios of means C ( max ) , AUC ( 0-t ) , AUC ( 0-infinity ) and T ( 1/2 ) all fell within the acceptance range of 0.8-1 .25 , demonstrating the bioequivalence of the two formulations .
	manualset3
152341	4	408129	13	NULL	NULL	0	NULL	means C ( max )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 90 % confidence intervals of the ratios of means C ( max ) , AUC ( 0-t ) , AUC ( 0-infinity ) and T ( 1/2 ) all fell within the acceptance range of 0.8-1 .25 , demonstrating the bioequivalence of the two formulations .
	manualset3
152342	5	408129	13	NULL	NULL	0	NULL	AUC ( 0-t )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 90 % confidence intervals of the ratios of means C ( max ) , AUC ( 0-t ) , AUC ( 0-infinity ) and T ( 1/2 ) all fell within the acceptance range of 0.8-1 .25 , demonstrating the bioequivalence of the two formulations .
	manualset3
152343	6	408129	13	NULL	NULL	0	NULL	AUC ( 0-infinity )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 90 % confidence intervals of the ratios of means C ( max ) , AUC ( 0-t ) , AUC ( 0-infinity ) and T ( 1/2 ) all fell within the acceptance range of 0.8-1 .25 , demonstrating the bioequivalence of the two formulations .
	manualset3
152344	7	408129	13	NULL	NULL	0	NULL	T ( 1/2 ) 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 90 % confidence intervals of the ratios of means C ( max ) , AUC ( 0-t ) , AUC ( 0-infinity ) and T ( 1/2 ) all fell within the acceptance range of 0.8-1 .25 , demonstrating the bioequivalence of the two formulations .
	manualset3
152345	8	408129	13	NULL	NULL	0	NULL	range 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 90 % confidence intervals of the ratios of means C ( max ) , AUC ( 0-t ) , AUC ( 0-infinity ) and T ( 1/2 ) all fell within the acceptance range of 0.8-1 .25 , demonstrating the bioequivalence of the two formulations .
	manualset3
152346	9	408129	13	NULL	NULL	0	NULL	0.8-1 .25 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 90 % confidence intervals of the ratios of means C ( max ) , AUC ( 0-t ) , AUC ( 0-infinity ) and T ( 1/2 ) all fell within the acceptance range of 0.8-1 .25 , demonstrating the bioequivalence of the two formulations .
	manualset3
152347	10	408129	13	NULL	NULL	0	NULL	bioequivalence	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The 90 % confidence intervals of the ratios of means C ( max ) , AUC ( 0-t ) , AUC ( 0-infinity ) and T ( 1/2 ) all fell within the acceptance range of 0.8-1 .25 , demonstrating the bioequivalence of the two formulations .
	manualset3
152348	11	408129	13	NULL	NULL	0	NULL	two formulations	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The 90 % confidence intervals of the ratios of means C ( max ) , AUC ( 0-t ) , AUC ( 0-infinity ) and T ( 1/2 ) all fell within the acceptance range of 0.8-1 .25 , demonstrating the bioequivalence of the two formulations .
	manualset3
152349	1	408130	13	NULL	NULL	0	NULL	AASI	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The AASI and its symmetric calculation ( Sym_AASI ) were derived from 24h-Ambulatory Blood Pressure Monitoring ( 24h-ABPM ) .
	manualset3
152350	2	408130	13	NULL	NULL	0	NULL	symmetric calculation ( Sym_AASI )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The AASI and its symmetric calculation ( Sym_AASI ) were derived from 24h-Ambulatory Blood Pressure Monitoring ( 24h-ABPM ) .
	manualset3
152351	3	408130	13	NULL	NULL	0	NULL	24h-Ambulatory Blood Pressure Monitoring ( 24h-ABPM ) 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The AASI and its symmetric calculation ( Sym_AASI ) were derived from 24h-Ambulatory Blood Pressure Monitoring ( 24h-ABPM ) .
	manualset3
152352	1	408131	13	NULL	NULL	0	NULL	ABP gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The ABP gene consisted of 5 exons and 4 introns and encoded a polypeptide of 198 residues .
	manualset3
152353	2	408131	13	NULL	NULL	0	NULL	5 exons	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The ABP gene consisted of 5 exons and 4 introns and encoded a polypeptide of 198 residues .
	manualset3
152354	3	408131	13	NULL	NULL	0	NULL	4 introns	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The ABP gene consisted of 5 exons and 4 introns and encoded a polypeptide of 198 residues .
	manualset3
152355	4	408131	13	NULL	NULL	0	NULL	polypeptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The ABP gene consisted of 5 exons and 4 introns and encoded a polypeptide of 198 residues .
	manualset3
152356	5	408131	13	NULL	NULL	0	NULL	198 residues	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The ABP gene consisted of 5 exons and 4 introns and encoded a polypeptide of 198 residues .
	manualset3
152357	1	408132	13	NULL	NULL	0	NULL	ACE insertion alleles 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The ACE insertion and deletion alleles had frequencies of 0.346 and 0.654 , respectively .
	manualset3
152358	2	408132	13	NULL	NULL	0	NULL	deletion alleles	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The ACE insertion and deletion alleles had frequencies of 0.346 and 0.654 , respectively .
	manualset3
152359	3	408132	13	NULL	NULL	0	NULL	frequencies 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ACE insertion and deletion alleles had frequencies of 0.346 and 0.654 , respectively .
	manualset3
152360	4	408132	13	NULL	NULL	0	NULL	0.346	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ACE insertion and deletion alleles had frequencies of 0.346 and 0.654 , respectively .
	manualset3
152361	5	408132	13	NULL	NULL	0	NULL	0.654	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ACE insertion and deletion alleles had frequencies of 0.346 and 0.654 , respectively .
	manualset3
152362	1	408133	13	NULL	NULL	0	NULL	AChE expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The AChE expression lags several days but follows roughly the same pattern of onset as for ChAT .
	manualset3
152363	2	408133	13	NULL	NULL	0	NULL	several days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The AChE expression lags several days but follows roughly the same pattern of onset as for ChAT .
	manualset3
152364	3	408133	13	NULL	NULL	0	NULL	pattern	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The AChE expression lags several days but follows roughly the same pattern of onset as for ChAT .
	manualset3
152365	4	408133	13	NULL	NULL	0	NULL	ChAT 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The AChE expression lags several days but follows roughly the same pattern of onset as for ChAT .
	manualset3
157277	5	408133	13	NULL	NULL	0	NULL	onset	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The AChE expression lags several days but follows roughly the same pattern of onset as for ChAT .
	manualset3
152366	1	408134	13	NULL	NULL	0	NULL	AGC family of protein kinases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The AGC family of protein kinases , which includes isoforms of protein kinase B ( also known as Akt ) , ribosomal S6 protein kinase ( S6K ) , and serum - and glucocorticoid-induced protein kinase ( SGK ) are activated in response to many extracellular signals and play key roles in regulating diverse cellular processes .
	manualset3
152367	2	408134	13	NULL	NULL	0	NULL	isoforms of protein kinase B	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The AGC family of protein kinases , which includes isoforms of protein kinase B ( also known as Akt ) , ribosomal S6 protein kinase ( S6K ) , and serum - and glucocorticoid-induced protein kinase ( SGK ) are activated in response to many extracellular signals and play key roles in regulating diverse cellular processes .
	manualset3
152368	3	408134	13	NULL	NULL	0	NULL	Akt	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The AGC family of protein kinases , which includes isoforms of protein kinase B ( also known as Akt ) , ribosomal S6 protein kinase ( S6K ) , and serum - and glucocorticoid-induced protein kinase ( SGK ) are activated in response to many extracellular signals and play key roles in regulating diverse cellular processes .
	manualset3
152369	4	408134	13	NULL	NULL	0	NULL	ribosomal S6 protein kinase ( S6K )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The AGC family of protein kinases , which includes isoforms of protein kinase B ( also known as Akt ) , ribosomal S6 protein kinase ( S6K ) , and serum - and glucocorticoid-induced protein kinase ( SGK ) are activated in response to many extracellular signals and play key roles in regulating diverse cellular processes .
	manualset3
152370	5	408134	13	NULL	NULL	0	NULL	serum - and glucocorticoid-induced protein kinase ( SGK )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The AGC family of protein kinases , which includes isoforms of protein kinase B ( also known as Akt ) , ribosomal S6 protein kinase ( S6K ) , and serum - and glucocorticoid-induced protein kinase ( SGK ) are activated in response to many extracellular signals and play key roles in regulating diverse cellular processes .
	manualset3
152371	6	408134	13	NULL	NULL	0	NULL	response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The AGC family of protein kinases , which includes isoforms of protein kinase B ( also known as Akt ) , ribosomal S6 protein kinase ( S6K ) , and serum - and glucocorticoid-induced protein kinase ( SGK ) are activated in response to many extracellular signals and play key roles in regulating diverse cellular processes .
	manualset3
152372	7	408134	13	NULL	NULL	0	NULL	extracellular signals	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The AGC family of protein kinases , which includes isoforms of protein kinase B ( also known as Akt ) , ribosomal S6 protein kinase ( S6K ) , and serum - and glucocorticoid-induced protein kinase ( SGK ) are activated in response to many extracellular signals and play key roles in regulating diverse cellular processes .
	manualset3
152373	8	408134	13	NULL	NULL	0	NULL	play key roles	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The AGC family of protein kinases , which includes isoforms of protein kinase B ( also known as Akt ) , ribosomal S6 protein kinase ( S6K ) , and serum - and glucocorticoid-induced protein kinase ( SGK ) are activated in response to many extracellular signals and play key roles in regulating diverse cellular processes .
	manualset3
152374	9	408134	13	NULL	NULL	0	NULL	cellular processes 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The AGC family of protein kinases , which includes isoforms of protein kinase B ( also known as Akt ) , ribosomal S6 protein kinase ( S6K ) , and serum - and glucocorticoid-induced protein kinase ( SGK ) are activated in response to many extracellular signals and play key roles in regulating diverse cellular processes .
	manualset3
152375	1	408135	13	NULL	NULL	NULL	NULL	AID	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The AID can not be corrected by acute infusions of glyburide or glipizide , or phentolamine , or by glycemic control after 2 weeks of intensive insulin treatments .
	manualset3
152376	2	408135	13	NULL	NULL	0	NULL	acute infusions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The AID can not be corrected by acute infusions of glyburide or glipizide , or phentolamine , or by glycemic control after 2 weeks of intensive insulin treatments .
	manualset3
152377	3	408135	13	NULL	NULL	0	NULL	glyburide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The AID can not be corrected by acute infusions of glyburide or glipizide , or phentolamine , or by glycemic control after 2 weeks of intensive insulin treatments .
	manualset3
152378	4	408135	13	NULL	NULL	0	NULL	glipizide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The AID can not be corrected by acute infusions of glyburide or glipizide , or phentolamine , or by glycemic control after 2 weeks of intensive insulin treatments .
	manualset3
152379	5	408135	13	NULL	NULL	0	NULL	phentolamine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The AID can not be corrected by acute infusions of glyburide or glipizide , or phentolamine , or by glycemic control after 2 weeks of intensive insulin treatments .
	manualset3
152380	6	408135	13	NULL	NULL	0	NULL	glycemic control	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The AID can not be corrected by acute infusions of glyburide or glipizide , or phentolamine , or by glycemic control after 2 weeks of intensive insulin treatments .
	manualset3
152381	7	408135	13	NULL	NULL	0	NULL	2 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The AID can not be corrected by acute infusions of glyburide or glipizide , or phentolamine , or by glycemic control after 2 weeks of intensive insulin treatments .
	manualset3
152382	8	408135	13	NULL	NULL	0	NULL	intensive insulin treatments	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The AID can not be corrected by acute infusions of glyburide or glipizide , or phentolamine , or by glycemic control after 2 weeks of intensive insulin treatments .
	manualset3
152383	1	408136	13	NULL	NULL	0	NULL	AMPLICOR system	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The AMPLICOR system correctly identified 94 ( 97.9 % ) of the 96 M. tuberculosis complex-positive MGITs and all 20 MAC-positive vials .
	manualset3
152384	2	408136	13	NULL	NULL	0	NULL	94	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The AMPLICOR system correctly identified 94 ( 97.9 % ) of the 96 M. tuberculosis complex-positive MGITs and all 20 MAC-positive vials .
	manualset3
152385	3	408136	13	NULL	NULL	0	NULL	97.9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The AMPLICOR system correctly identified 94 ( 97.9 % ) of the 96 M. tuberculosis complex-positive MGITs and all 20 MAC-positive vials .
	manualset3
152386	4	408136	13	NULL	NULL	0	NULL	96	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The AMPLICOR system correctly identified 94 ( 97.9 % ) of the 96 M. tuberculosis complex-positive MGITs and all 20 MAC-positive vials .
	manualset3
152387	5	408136	13	NULL	NULL	NULL	NULL	M. tuberculosis complex-positive MGITs	Thing												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The AMPLICOR system correctly identified 94 ( 97.9 % ) of the 96 M. tuberculosis complex-positive MGITs and all 20 MAC-positive vials .
	manualset3
152388	6	408136	13	NULL	NULL	0	NULL	 20 MAC-positive vials	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The AMPLICOR system correctly identified 94 ( 97.9 % ) of the 96 M. tuberculosis complex-positive MGITs and all 20 MAC-positive vials .
	manualset3
152389	1	408137	13	NULL	NULL	0	NULL	50 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ANF-induced 50 % decreased CGRP excretion occurred after the circulating concentration of CGRP had returned to preinfusion levels .
	manualset3
152390	2	408137	13	NULL	NULL	0	NULL	CGRP excretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ANF-induced 50 % decreased CGRP excretion occurred after the circulating concentration of CGRP had returned to preinfusion levels .
	manualset3
152391	3	408137	13	NULL	NULL	0	NULL	concentration 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ANF-induced 50 % decreased CGRP excretion occurred after the circulating concentration of CGRP had returned to preinfusion levels .
	manualset3
152392	4	408137	13	NULL	NULL	0	NULL	CGRP	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The ANF-induced 50 % decreased CGRP excretion occurred after the circulating concentration of CGRP had returned to preinfusion levels .
	manualset3
152393	5	408137	13	NULL	NULL	0	NULL	preinfusion levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ANF-induced 50 % decreased CGRP excretion occurred after the circulating concentration of CGRP had returned to preinfusion levels .
	manualset3
152394	1	408138	13	NULL	NULL	0	NULL	APC tumor suppressor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The APC tumor suppressor contributes to chromosome segregation and turnover of the oncogenic transcriptional activator beta-catenin , and these activities are impaired by truncating cancer mutations .
	manualset3
152395	2	408138	13	NULL	NULL	0	NULL	chromosome segregation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The APC tumor suppressor contributes to chromosome segregation and turnover of the oncogenic transcriptional activator beta-catenin , and these activities are impaired by truncating cancer mutations .
	manualset3
152396	3	408138	13	NULL	NULL	0	NULL	turnover	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The APC tumor suppressor contributes to chromosome segregation and turnover of the oncogenic transcriptional activator beta-catenin , and these activities are impaired by truncating cancer mutations .
	manualset3
152397	4	408138	13	NULL	NULL	0	NULL	oncogenic transcriptional activator beta-catenin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The APC tumor suppressor contributes to chromosome segregation and turnover of the oncogenic transcriptional activator beta-catenin , and these activities are impaired by truncating cancer mutations .
	manualset3
152398	5	408138	13	NULL	NULL	0	NULL	activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The APC tumor suppressor contributes to chromosome segregation and turnover of the oncogenic transcriptional activator beta-catenin , and these activities are impaired by truncating cancer mutations .
	manualset3
152399	6	408138	13	NULL	NULL	0	NULL	cancer mutations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The APC tumor suppressor contributes to chromosome segregation and turnover of the oncogenic transcriptional activator beta-catenin , and these activities are impaired by truncating cancer mutations .
	manualset3
152400	1	408139	13	NULL	NULL	0	NULL	distribution of mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A random distribution of mutations affecting splice acceptor sites ( 22 % ) was induced by ( + / - ) - syn-BgCDE .
	manualset3
152401	2	408139	13	NULL	NULL	0	NULL	splice acceptor sites	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A random distribution of mutations affecting splice acceptor sites ( 22 % ) was induced by ( + / - ) - syn-BgCDE .
	manualset3
152402	3	408139	13	NULL	NULL	0	NULL	 22 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A random distribution of mutations affecting splice acceptor sites ( 22 % ) was induced by ( + / - ) - syn-BgCDE .
	manualset3
152403	4	408139	13	NULL	NULL	0	NULL	( + / - ) - syn-BgCDE	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A random distribution of mutations affecting splice acceptor sites ( 22 % ) was induced by ( + / - ) - syn-BgCDE .
	manualset3
152404	1	408140	13	NULL	NULL	0	NULL	ATP-dependent 45Ca2 + uptake 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ATP-dependent 45Ca2 + uptake by inside-out plasma-membrane vesicles was about 20 times more sensitive to saponin than was the ATP-dependent uptake by a microsomal preparation .
	manualset3
152405	2	408140	13	NULL	NULL	0	NULL	plasma-membrane vesicles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The ATP-dependent 45Ca2 + uptake by inside-out plasma-membrane vesicles was about 20 times more sensitive to saponin than was the ATP-dependent uptake by a microsomal preparation .
	manualset3
152406	3	408140	13	NULL	NULL	0	NULL	20 times	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ATP-dependent 45Ca2 + uptake by inside-out plasma-membrane vesicles was about 20 times more sensitive to saponin than was the ATP-dependent uptake by a microsomal preparation .
	manualset3
152407	4	408140	13	NULL	NULL	0	NULL	saponin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ATP-dependent 45Ca2 + uptake by inside-out plasma-membrane vesicles was about 20 times more sensitive to saponin than was the ATP-dependent uptake by a microsomal preparation .
	manualset3
152408	5	408140	13	NULL	NULL	0	NULL	ATP-dependent uptake	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ATP-dependent 45Ca2 + uptake by inside-out plasma-membrane vesicles was about 20 times more sensitive to saponin than was the ATP-dependent uptake by a microsomal preparation .
	manualset3
152409	6	408140	13	NULL	NULL	0	NULL	microsomal preparation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ATP-dependent 45Ca2 + uptake by inside-out plasma-membrane vesicles was about 20 times more sensitive to saponin than was the ATP-dependent uptake by a microsomal preparation .
	manualset3
152410	1	408141	13	NULL	NULL	0	NULL	AVP response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The AVP response was severely impaired by DSAP .
	manualset3
152411	2	408141	13	NULL	NULL	0	NULL	DSAP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The AVP response was severely impaired by DSAP .
	manualset3
152412	1	408142	13	NULL	NULL	NULL	NULL	Acute Coronary Syndrome 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The Acute Coronary Syndrome Prospective Audit is a prospective multicenter registry with 12-month outcome data for 3 , 393 patients ( 755 with ST-segment elevation myocardial infarction , 1942 with high-risk non-ST-segment elevation ACS ( NSTE-ACS ) , and 696 with intermediate-risk NSTE-ACS ) .
	manualset3
152413	3	408142	13	NULL	NULL	NULL	NULL	multicenter registry	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The Acute Coronary Syndrome Prospective Audit is a prospective multicenter registry with 12-month outcome data for 3 , 393 patients ( 755 with ST-segment elevation myocardial infarction , 1942 with high-risk non-ST-segment elevation ACS ( NSTE-ACS ) , and 696 with intermediate-risk NSTE-ACS ) .
	manualset3
152414	4	408142	13	NULL	NULL	NULL	NULL	12-month	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The Acute Coronary Syndrome Prospective Audit is a prospective multicenter registry with 12-month outcome data for 3 , 393 patients ( 755 with ST-segment elevation myocardial infarction , 1942 with high-risk non-ST-segment elevation ACS ( NSTE-ACS ) , and 696 with intermediate-risk NSTE-ACS ) .
	manualset3
152415	2	408142	13	NULL	NULL	0	NULL	Audit 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Acute Coronary Syndrome Prospective Audit is a prospective multicenter registry with 12-month outcome data for 3 , 393 patients ( 755 with ST-segment elevation myocardial infarction , 1942 with high-risk non-ST-segment elevation ACS ( NSTE-ACS ) , and 696 with intermediate-risk NSTE-ACS ) .
	manualset3
152416	5	408142	13	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The Acute Coronary Syndrome Prospective Audit is a prospective multicenter registry with 12-month outcome data for 3 , 393 patients ( 755 with ST-segment elevation myocardial infarction , 1942 with high-risk non-ST-segment elevation ACS ( NSTE-ACS ) , and 696 with intermediate-risk NSTE-ACS ) .
	manualset3
152417	6	408142	13	NULL	NULL	0	NULL	3 , 393 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The Acute Coronary Syndrome Prospective Audit is a prospective multicenter registry with 12-month outcome data for 3 , 393 patients ( 755 with ST-segment elevation myocardial infarction , 1942 with high-risk non-ST-segment elevation ACS ( NSTE-ACS ) , and 696 with intermediate-risk NSTE-ACS ) .
	manualset3
152418	7	408142	13	NULL	NULL	0	NULL	755	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Acute Coronary Syndrome Prospective Audit is a prospective multicenter registry with 12-month outcome data for 3 , 393 patients ( 755 with ST-segment elevation myocardial infarction , 1942 with high-risk non-ST-segment elevation ACS ( NSTE-ACS ) , and 696 with intermediate-risk NSTE-ACS ) .
	manualset3
152419	8	408142	13	NULL	NULL	0	NULL	ST-segment elevation myocardial infarction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Acute Coronary Syndrome Prospective Audit is a prospective multicenter registry with 12-month outcome data for 3 , 393 patients ( 755 with ST-segment elevation myocardial infarction , 1942 with high-risk non-ST-segment elevation ACS ( NSTE-ACS ) , and 696 with intermediate-risk NSTE-ACS ) .
	manualset3
152420	9	408142	13	NULL	NULL	0	NULL	1942 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Acute Coronary Syndrome Prospective Audit is a prospective multicenter registry with 12-month outcome data for 3 , 393 patients ( 755 with ST-segment elevation myocardial infarction , 1942 with high-risk non-ST-segment elevation ACS ( NSTE-ACS ) , and 696 with intermediate-risk NSTE-ACS ) .
	manualset3
152421	10	408142	13	NULL	NULL	0	NULL	high-risk non-ST-segment elevation ACS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Acute Coronary Syndrome Prospective Audit is a prospective multicenter registry with 12-month outcome data for 3 , 393 patients ( 755 with ST-segment elevation myocardial infarction , 1942 with high-risk non-ST-segment elevation ACS ( NSTE-ACS ) , and 696 with intermediate-risk NSTE-ACS ) .
	manualset3
152422	11	408142	13	NULL	NULL	0	NULL	NSTE-ACS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Acute Coronary Syndrome Prospective Audit is a prospective multicenter registry with 12-month outcome data for 3 , 393 patients ( 755 with ST-segment elevation myocardial infarction , 1942 with high-risk non-ST-segment elevation ACS ( NSTE-ACS ) , and 696 with intermediate-risk NSTE-ACS ) .
	manualset3
152423	12	408142	13	NULL	NULL	0	NULL	696 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Acute Coronary Syndrome Prospective Audit is a prospective multicenter registry with 12-month outcome data for 3 , 393 patients ( 755 with ST-segment elevation myocardial infarction , 1942 with high-risk non-ST-segment elevation ACS ( NSTE-ACS ) , and 696 with intermediate-risk NSTE-ACS ) .
	manualset3
152424	13	408142	13	NULL	NULL	0	NULL	 intermediate-risk NSTE-ACS ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Acute Coronary Syndrome Prospective Audit is a prospective multicenter registry with 12-month outcome data for 3 , 393 patients ( 755 with ST-segment elevation myocardial infarction , 1942 with high-risk non-ST-segment elevation ACS ( NSTE-ACS ) , and 696 with intermediate-risk NSTE-ACS ) .
	manualset3
152425	1	408143	13	NULL	NULL	0	NULL	Ala	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The Ala and Asn replacements have a profound effect on the exonuclease activity of T4 DNA polymerase and also have a significant , but less pronounced influence on its polymerase activity which is located in a domain distal to the exonuclease region .
	manualset3
152426	2	408143	13	NULL	NULL	0	NULL	Asn	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The Ala and Asn replacements have a profound effect on the exonuclease activity of T4 DNA polymerase and also have a significant , but less pronounced influence on its polymerase activity which is located in a domain distal to the exonuclease region .
	manualset3
152427	3	408143	13	NULL	NULL	0	NULL	replacements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Ala and Asn replacements have a profound effect on the exonuclease activity of T4 DNA polymerase and also have a significant , but less pronounced influence on its polymerase activity which is located in a domain distal to the exonuclease region .
	manualset3
152428	4	408143	13	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Ala and Asn replacements have a profound effect on the exonuclease activity of T4 DNA polymerase and also have a significant , but less pronounced influence on its polymerase activity which is located in a domain distal to the exonuclease region .
	manualset3
152429	5	408143	13	NULL	NULL	0	NULL	exonuclease activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Ala and Asn replacements have a profound effect on the exonuclease activity of T4 DNA polymerase and also have a significant , but less pronounced influence on its polymerase activity which is located in a domain distal to the exonuclease region .
	manualset3
152430	6	408143	13	NULL	NULL	0	NULL	T4 DNA polymerase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The Ala and Asn replacements have a profound effect on the exonuclease activity of T4 DNA polymerase and also have a significant , but less pronounced influence on its polymerase activity which is located in a domain distal to the exonuclease region .
	manualset3
152431	7	408143	13	NULL	NULL	0	NULL	influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Ala and Asn replacements have a profound effect on the exonuclease activity of T4 DNA polymerase and also have a significant , but less pronounced influence on its polymerase activity which is located in a domain distal to the exonuclease region .
	manualset3
152432	8	408143	13	NULL	NULL	0	NULL	polymerase activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Ala and Asn replacements have a profound effect on the exonuclease activity of T4 DNA polymerase and also have a significant , but less pronounced influence on its polymerase activity which is located in a domain distal to the exonuclease region .
	manualset3
152433	9	408143	13	NULL	NULL	0	NULL	domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The Ala and Asn replacements have a profound effect on the exonuclease activity of T4 DNA polymerase and also have a significant , but less pronounced influence on its polymerase activity which is located in a domain distal to the exonuclease region .
	manualset3
152434	10	408143	13	NULL	NULL	0	NULL	exonuclease region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The Ala and Asn replacements have a profound effect on the exonuclease activity of T4 DNA polymerase and also have a significant , but less pronounced influence on its polymerase activity which is located in a domain distal to the exonuclease region .
	manualset3
152435	1	408144	13	NULL	NULL	0	NULL	American Dietetic Association position paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The American Dietetic Association position paper on bland diet in the treatment of chronic duodenal ulcer disease .
	manualset3
152436	2	408144	13	NULL	NULL	0	NULL	bland diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The American Dietetic Association position paper on bland diet in the treatment of chronic duodenal ulcer disease .
	manualset3
152437	3	408144	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The American Dietetic Association position paper on bland diet in the treatment of chronic duodenal ulcer disease .
	manualset3
152438	4	408144	13	NULL	NULL	0	NULL	chronic duodenal ulcer disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The American Dietetic Association position paper on bland diet in the treatment of chronic duodenal ulcer disease .
	manualset3
152439	1	408145	13	NULL	NULL	0	NULL	Arabidopsis J-domain proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The Arabidopsis J-domain proteins ARG1 and ARL2 function as gravity-signal transducers in root statocytes .
	manualset3
152440	2	408145	13	NULL	NULL	0	NULL	ARG1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The Arabidopsis J-domain proteins ARG1 and ARL2 function as gravity-signal transducers in root statocytes .
	manualset3
152441	3	408145	13	NULL	NULL	0	NULL	ARL2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The Arabidopsis J-domain proteins ARG1 and ARL2 function as gravity-signal transducers in root statocytes .
	manualset3
152442	4	408145	13	NULL	NULL	0	NULL	function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Arabidopsis J-domain proteins ARG1 and ARL2 function as gravity-signal transducers in root statocytes .
	manualset3
152443	5	408145	13	NULL	NULL	0	NULL	gravity-signal transducers	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The Arabidopsis J-domain proteins ARG1 and ARL2 function as gravity-signal transducers in root statocytes .
	manualset3
152444	6	408145	13	NULL	NULL	0	NULL	root statocytes	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The Arabidopsis J-domain proteins ARG1 and ARL2 function as gravity-signal transducers in root statocytes .
	manualset3
152445	1	408146	13	NULL	NULL	0	NULL	Arctic Medicine Conference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Arctic Medicine Conference is a medical conference with talks in Zoonoses , Dentistry , Entomology , and Travel Medicine hosted by Wilderness Medicine in Manitoba ( www.skylarkmedicalclinic.com ) .
	manualset3
152446	2	408146	13	NULL	NULL	0	NULL	medical conference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Arctic Medicine Conference is a medical conference with talks in Zoonoses , Dentistry , Entomology , and Travel Medicine hosted by Wilderness Medicine in Manitoba ( www.skylarkmedicalclinic.com ) .
	manualset3
152447	3	408146	13	NULL	NULL	0	NULL	 talks	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Arctic Medicine Conference is a medical conference with talks in Zoonoses , Dentistry , Entomology , and Travel Medicine hosted by Wilderness Medicine in Manitoba ( www.skylarkmedicalclinic.com ) .
	manualset3
152448	4	408146	13	NULL	NULL	0	NULL	Zoonoses 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The Arctic Medicine Conference is a medical conference with talks in Zoonoses , Dentistry , Entomology , and Travel Medicine hosted by Wilderness Medicine in Manitoba ( www.skylarkmedicalclinic.com ) .
	manualset3
152449	5	408146	13	NULL	NULL	0	NULL	Dentistry	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The Arctic Medicine Conference is a medical conference with talks in Zoonoses , Dentistry , Entomology , and Travel Medicine hosted by Wilderness Medicine in Manitoba ( www.skylarkmedicalclinic.com ) .
	manualset3
152450	6	408146	13	NULL	NULL	0	NULL	Entomology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The Arctic Medicine Conference is a medical conference with talks in Zoonoses , Dentistry , Entomology , and Travel Medicine hosted by Wilderness Medicine in Manitoba ( www.skylarkmedicalclinic.com ) .
	manualset3
152451	7	408146	13	NULL	NULL	0	NULL	Travel Medicine	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The Arctic Medicine Conference is a medical conference with talks in Zoonoses , Dentistry , Entomology , and Travel Medicine hosted by Wilderness Medicine in Manitoba ( www.skylarkmedicalclinic.com ) .
	manualset3
152452	8	408146	13	NULL	NULL	0	NULL	Wilderness Medicine	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The Arctic Medicine Conference is a medical conference with talks in Zoonoses , Dentistry , Entomology , and Travel Medicine hosted by Wilderness Medicine in Manitoba ( www.skylarkmedicalclinic.com ) .
	manualset3
152453	9	408146	13	NULL	NULL	0	NULL	Manitoba	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The Arctic Medicine Conference is a medical conference with talks in Zoonoses , Dentistry , Entomology , and Travel Medicine hosted by Wilderness Medicine in Manitoba ( www.skylarkmedicalclinic.com ) .
	manualset3
152454	1	408147	13	NULL	NULL	0	NULL	sample	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A random sample of 2 , 053 residents of San Diego , CA , were surveyed regarding exercise habits and other variables .
	manualset3
152455	2	408147	13	NULL	NULL	0	NULL	2 , 053 residents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A random sample of 2 , 053 residents of San Diego , CA , were surveyed regarding exercise habits and other variables .
	manualset3
152456	3	408147	13	NULL	NULL	0	NULL	San Diego	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A random sample of 2 , 053 residents of San Diego , CA , were surveyed regarding exercise habits and other variables .
	manualset3
152457	4	408147	13	NULL	NULL	0	NULL	CA	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A random sample of 2 , 053 residents of San Diego , CA , were surveyed regarding exercise habits and other variables .
	manualset3
152458	5	408147	13	NULL	NULL	0	NULL	exercise habits	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A random sample of 2 , 053 residents of San Diego , CA , were surveyed regarding exercise habits and other variables .
	manualset3
152459	6	408147	13	NULL	NULL	0	NULL	variables	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A random sample of 2 , 053 residents of San Diego , CA , were surveyed regarding exercise habits and other variables .
	manualset3
152460	1	408148	13	NULL	NULL	0	NULL	Arf/p53 pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Arf/p53 pathway protects cells against several types of damage and this is the basis of its tumor suppressor activity .
	manualset3
152461	2	408148	13	NULL	NULL	0	NULL	cells	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The Arf/p53 pathway protects cells against several types of damage and this is the basis of its tumor suppressor activity .
	manualset3
152462	3	408148	13	NULL	NULL	0	NULL	types of damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Arf/p53 pathway protects cells against several types of damage and this is the basis of its tumor suppressor activity .
	manualset3
152463	4	408148	13	NULL	NULL	0	NULL	basis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Arf/p53 pathway protects cells against several types of damage and this is the basis of its tumor suppressor activity .
	manualset3
152464	5	408148	13	NULL	NULL	0	NULL	tumor suppressor activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Arf/p53 pathway protects cells against several types of damage and this is the basis of its tumor suppressor activity .
	manualset3
152465	1	408149	13	NULL	NULL	0	NULL	AttHRV/VLP2x regimen	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The AttHRV/VLP2x regimen stimulated the highest mean numbers of intestinal immunoglobulin A ( IgA ) ASCs prechallenge among all vaccine groups .
	manualset3
152466	2	408149	13	NULL	NULL	0	NULL	mean numbers	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The AttHRV/VLP2x regimen stimulated the highest mean numbers of intestinal immunoglobulin A ( IgA ) ASCs prechallenge among all vaccine groups .
	manualset3
152467	3	408149	13	NULL	NULL	0	NULL	intestinal immunoglobulin A ( IgA ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The AttHRV/VLP2x regimen stimulated the highest mean numbers of intestinal immunoglobulin A ( IgA ) ASCs prechallenge among all vaccine groups .
	manualset3
152468	4	408149	13	NULL	NULL	0	NULL	ASCs	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The AttHRV/VLP2x regimen stimulated the highest mean numbers of intestinal immunoglobulin A ( IgA ) ASCs prechallenge among all vaccine groups .
	manualset3
152469	5	408149	13	NULL	NULL	0	NULL	prechallenge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The AttHRV/VLP2x regimen stimulated the highest mean numbers of intestinal immunoglobulin A ( IgA ) ASCs prechallenge among all vaccine groups .
	manualset3
152470	6	408149	13	NULL	NULL	0	NULL	vaccine groups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The AttHRV/VLP2x regimen stimulated the highest mean numbers of intestinal immunoglobulin A ( IgA ) ASCs prechallenge among all vaccine groups .
	manualset3
152471	1	408150	13	NULL	NULL	0	NULL	B-scan 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The B-scan was superior to the A-scan .
	manualset3
152472	2	408150	13	NULL	NULL	0	NULL	A-scan 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The B-scan was superior to the A-scan .
	manualset3
152473	1	408151	13	NULL	NULL	0	NULL	BCL6 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The BCL6 gene , which encodes a zinc-finger transcription repressor protein and which maps to chromosomal band 3q27 , is deregulated in t ( 3 ; 14 ) ( q27 ; q32 ) and other translocations by substitution of its transcription regulatory sequences by those of genes on the partner chromosomes .
	manualset3
152474	2	408151	13	NULL	NULL	0	NULL	zinc-finger transcription repressor protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The BCL6 gene , which encodes a zinc-finger transcription repressor protein and which maps to chromosomal band 3q27 , is deregulated in t ( 3 ; 14 ) ( q27 ; q32 ) and other translocations by substitution of its transcription regulatory sequences by those of genes on the partner chromosomes .
	manualset3
152475	3	408151	13	NULL	NULL	0	NULL	maps 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The BCL6 gene , which encodes a zinc-finger transcription repressor protein and which maps to chromosomal band 3q27 , is deregulated in t ( 3 ; 14 ) ( q27 ; q32 ) and other translocations by substitution of its transcription regulatory sequences by those of genes on the partner chromosomes .
	manualset3
152476	4	408151	13	NULL	NULL	0	NULL	chromosomal band 3q27	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The BCL6 gene , which encodes a zinc-finger transcription repressor protein and which maps to chromosomal band 3q27 , is deregulated in t ( 3 ; 14 ) ( q27 ; q32 ) and other translocations by substitution of its transcription regulatory sequences by those of genes on the partner chromosomes .
	manualset3
152477	5	408151	13	NULL	NULL	0	NULL	 t ( 3 ; 14 ) ( q27 ; q32 ) 	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The BCL6 gene , which encodes a zinc-finger transcription repressor protein and which maps to chromosomal band 3q27 , is deregulated in t ( 3 ; 14 ) ( q27 ; q32 ) and other translocations by substitution of its transcription regulatory sequences by those of genes on the partner chromosomes .
	manualset3
152478	6	408151	13	NULL	NULL	0	NULL	translocations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The BCL6 gene , which encodes a zinc-finger transcription repressor protein and which maps to chromosomal band 3q27 , is deregulated in t ( 3 ; 14 ) ( q27 ; q32 ) and other translocations by substitution of its transcription regulatory sequences by those of genes on the partner chromosomes .
	manualset3
152479	7	408151	13	NULL	NULL	0	NULL	substitution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The BCL6 gene , which encodes a zinc-finger transcription repressor protein and which maps to chromosomal band 3q27 , is deregulated in t ( 3 ; 14 ) ( q27 ; q32 ) and other translocations by substitution of its transcription regulatory sequences by those of genes on the partner chromosomes .
	manualset3
152480	8	408151	13	NULL	NULL	0	NULL	transcription regulatory sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The BCL6 gene , which encodes a zinc-finger transcription repressor protein and which maps to chromosomal band 3q27 , is deregulated in t ( 3 ; 14 ) ( q27 ; q32 ) and other translocations by substitution of its transcription regulatory sequences by those of genes on the partner chromosomes .
	manualset3
152481	9	408151	13	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The BCL6 gene , which encodes a zinc-finger transcription repressor protein and which maps to chromosomal band 3q27 , is deregulated in t ( 3 ; 14 ) ( q27 ; q32 ) and other translocations by substitution of its transcription regulatory sequences by those of genes on the partner chromosomes .
	manualset3
152482	10	408151	13	NULL	NULL	0	NULL	partner chromosomes 	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The BCL6 gene , which encodes a zinc-finger transcription repressor protein and which maps to chromosomal band 3q27 , is deregulated in t ( 3 ; 14 ) ( q27 ; q32 ) and other translocations by substitution of its transcription regulatory sequences by those of genes on the partner chromosomes .
	manualset3
152483	1	408152	13	NULL	NULL	0	NULL	BCL6 proto-oncogene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The BCL6 proto-oncogene encodes a transcriptional repressor necessary for the development of germinal centers ( GCs ) and directly implicated in lymphomagenesis .
	manualset3
152484	2	408152	13	NULL	NULL	0	NULL	transcriptional repressor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The BCL6 proto-oncogene encodes a transcriptional repressor necessary for the development of germinal centers ( GCs ) and directly implicated in lymphomagenesis .
	manualset3
152485	3	408152	13	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The BCL6 proto-oncogene encodes a transcriptional repressor necessary for the development of germinal centers ( GCs ) and directly implicated in lymphomagenesis .
	manualset3
152486	4	408152	13	NULL	NULL	0	NULL	germinal centers ( GCs ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The BCL6 proto-oncogene encodes a transcriptional repressor necessary for the development of germinal centers ( GCs ) and directly implicated in lymphomagenesis .
	manualset3
152487	5	408152	13	NULL	NULL	0	NULL	lymphomagenesis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The BCL6 proto-oncogene encodes a transcriptional repressor necessary for the development of germinal centers ( GCs ) and directly implicated in lymphomagenesis .
	manualset3
152488	1	408153	13	NULL	NULL	0	NULL	BI birds	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The BI birds had significantly fewer leg abnormalities than E birds .
	manualset3
152489	2	408153	13	NULL	NULL	0	NULL	leg abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The BI birds had significantly fewer leg abnormalities than E birds .
	manualset3
152490	3	408153	13	NULL	NULL	0	NULL	E birds	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The BI birds had significantly fewer leg abnormalities than E birds .
	manualset3
152491	1	408154	13	NULL	NULL	0	NULL	BIRN	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The BIRN is a multi-university consortium collaborating to establish a large-scale data and computational grid around neuroimaging data , collected across multiple scales .
	manualset3
152492	2	408154	13	NULL	NULL	0	NULL	multi-university consortium	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The BIRN is a multi-university consortium collaborating to establish a large-scale data and computational grid around neuroimaging data , collected across multiple scales .
	manualset3
152493	3	408154	13	NULL	NULL	0	NULL	large-scale data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The BIRN is a multi-university consortium collaborating to establish a large-scale data and computational grid around neuroimaging data , collected across multiple scales .
	manualset3
152494	4	408154	13	NULL	NULL	0	NULL	computational grid	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The BIRN is a multi-university consortium collaborating to establish a large-scale data and computational grid around neuroimaging data , collected across multiple scales .
	manualset3
152495	5	408154	13	NULL	NULL	0	NULL	neuroimaging data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The BIRN is a multi-university consortium collaborating to establish a large-scale data and computational grid around neuroimaging data , collected across multiple scales .
	manualset3
152496	6	408154	13	NULL	NULL	0	NULL	multiple scales	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The BIRN is a multi-university consortium collaborating to establish a large-scale data and computational grid around neuroimaging data , collected across multiple scales .
	manualset3
152497	1	408155	13	NULL	NULL	0	NULL	BMI method	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The BMI method confirmed that DAKG is taken up by the brain to rapidly release ketoprofen in a dose-dependent manner .
	manualset3
152498	2	408155	13	NULL	NULL	0	NULL	DAKG	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The BMI method confirmed that DAKG is taken up by the brain to rapidly release ketoprofen in a dose-dependent manner .
	manualset3
152499	3	408155	13	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The BMI method confirmed that DAKG is taken up by the brain to rapidly release ketoprofen in a dose-dependent manner .
	manualset3
152501	4	408155	13	NULL	NULL	NULL	NULL	ketoprofen	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The BMI method confirmed that DAKG is taken up by the brain to rapidly release ketoprofen in a dose-dependent manner .
	manualset3
152502	5	408155	13	NULL	NULL	0	NULL	dose-dependent manner	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The BMI method confirmed that DAKG is taken up by the brain to rapidly release ketoprofen in a dose-dependent manner .
	manualset3
152503	1	408156	13	NULL	NULL	0	NULL	BTAi 1 isolate 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The BTAi 1 isolate can be differentiated from members of the family Rhodospirillaceae by several criteria .
	manualset3
152504	2	408156	13	NULL	NULL	0	NULL	members	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The BTAi 1 isolate can be differentiated from members of the family Rhodospirillaceae by several criteria .
	manualset3
152505	3	408156	13	NULL	NULL	0	NULL	family Rhodospirillaceae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The BTAi 1 isolate can be differentiated from members of the family Rhodospirillaceae by several criteria .
	manualset3
152506	4	408156	13	NULL	NULL	0	NULL	several criteria 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The BTAi 1 isolate can be differentiated from members of the family Rhodospirillaceae by several criteria .
	manualset3
152507	1	408157	13	NULL	NULL	0	NULL	 random sample	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A random sample of 72 children , 5 to 17 years old , with doctor-diagnosed asthma who lived in the same residence ) or = 2 years were enrolled .
	manualset3
152508	2	408157	13	NULL	NULL	0	NULL	72 children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A random sample of 72 children , 5 to 17 years old , with doctor-diagnosed asthma who lived in the same residence ) or = 2 years were enrolled .
	manualset3
152509	3	408157	13	NULL	NULL	0	NULL	5 to 17 years old 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A random sample of 72 children , 5 to 17 years old , with doctor-diagnosed asthma who lived in the same residence ) or = 2 years were enrolled .
	manualset3
152510	4	408157	13	NULL	NULL	0	NULL	asthma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A random sample of 72 children , 5 to 17 years old , with doctor-diagnosed asthma who lived in the same residence ) or = 2 years were enrolled .
	manualset3
152511	5	408157	13	NULL	NULL	0	NULL	residence 	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A random sample of 72 children , 5 to 17 years old , with doctor-diagnosed asthma who lived in the same residence ) or = 2 years were enrolled .
	manualset3
152512	6	408157	13	NULL	NULL	0	NULL	2 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A random sample of 72 children , 5 to 17 years old , with doctor-diagnosed asthma who lived in the same residence ) or = 2 years were enrolled .
	manualset3
152513	1	408158	13	NULL	NULL	0	NULL	Bingeing 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Bingeing and Eating cues scale was negatively associated with program attendance .
	manualset3
152514	2	408158	13	NULL	NULL	0	NULL	Eating cues scale	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Bingeing and Eating cues scale was negatively associated with program attendance .
	manualset3
152515	3	408158	13	NULL	NULL	0	NULL	program attendance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Bingeing and Eating cues scale was negatively associated with program attendance .
	manualset3
152516	1	408159	13	NULL	NULL	0	NULL	 Blec4 promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The Blec4 promoter represents a useful tool with which to target the expression of foreign genes to the epidermal layer of actively growing shoots .
	manualset3
152517	2	408159	13	NULL	NULL	0	NULL	tool	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The Blec4 promoter represents a useful tool with which to target the expression of foreign genes to the epidermal layer of actively growing shoots .
	manualset3
152519	4	408159	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Blec4 promoter represents a useful tool with which to target the expression of foreign genes to the epidermal layer of actively growing shoots .
	manualset3
152520	5	408159	13	NULL	NULL	0	NULL	foreign genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The Blec4 promoter represents a useful tool with which to target the expression of foreign genes to the epidermal layer of actively growing shoots .
	manualset3
152521	6	408159	13	NULL	NULL	0	NULL	epidermal layer	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The Blec4 promoter represents a useful tool with which to target the expression of foreign genes to the epidermal layer of actively growing shoots .
	manualset3
152522	7	408159	13	NULL	NULL	0	NULL	shoots	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The Blec4 promoter represents a useful tool with which to target the expression of foreign genes to the epidermal layer of actively growing shoots .
	manualset3
152523	1	408160	13	NULL	NULL	0	NULL	Bow Creek watershed	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The Bow Creek watershed ( Nebraska , USA ) is dominated by the production of beef cattle and row crops ; therefore , surface waters are likely to receive runoff containing steroid hormones and pesticides .
	manualset3
152524	2	408160	13	NULL	NULL	0	NULL	Nebraska , USA 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The Bow Creek watershed ( Nebraska , USA ) is dominated by the production of beef cattle and row crops ; therefore , surface waters are likely to receive runoff containing steroid hormones and pesticides .
	manualset3
152525	3	408160	13	NULL	NULL	0	NULL	production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Bow Creek watershed ( Nebraska , USA ) is dominated by the production of beef cattle and row crops ; therefore , surface waters are likely to receive runoff containing steroid hormones and pesticides .
	manualset3
152526	4	408160	13	NULL	NULL	0	NULL	beef cattle	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The Bow Creek watershed ( Nebraska , USA ) is dominated by the production of beef cattle and row crops ; therefore , surface waters are likely to receive runoff containing steroid hormones and pesticides .
	manualset3
152527	5	408160	13	NULL	NULL	0	NULL	row crops	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The Bow Creek watershed ( Nebraska , USA ) is dominated by the production of beef cattle and row crops ; therefore , surface waters are likely to receive runoff containing steroid hormones and pesticides .
	manualset3
152528	6	408160	13	NULL	NULL	0	NULL	surface waters	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The Bow Creek watershed ( Nebraska , USA ) is dominated by the production of beef cattle and row crops ; therefore , surface waters are likely to receive runoff containing steroid hormones and pesticides .
	manualset3
152529	7	408160	13	NULL	NULL	0	NULL	runoff	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Bow Creek watershed ( Nebraska , USA ) is dominated by the production of beef cattle and row crops ; therefore , surface waters are likely to receive runoff containing steroid hormones and pesticides .
	manualset3
152530	8	408160	13	NULL	NULL	0	NULL	steroid hormones 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The Bow Creek watershed ( Nebraska , USA ) is dominated by the production of beef cattle and row crops ; therefore , surface waters are likely to receive runoff containing steroid hormones and pesticides .
	manualset3
152531	9	408160	13	NULL	NULL	0	NULL	pesticides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The Bow Creek watershed ( Nebraska , USA ) is dominated by the production of beef cattle and row crops ; therefore , surface waters are likely to receive runoff containing steroid hormones and pesticides .
	manualset3
152532	1	408161	13	NULL	NULL	0	NULL	Brunham model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The Brunham model is an important attempt to model the effects of different assumptions about rates of partner exchange on disease prevalence and on sterility levels .
	manualset3
152533	2	408161	13	NULL	NULL	0	NULL	attempt	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Brunham model is an important attempt to model the effects of different assumptions about rates of partner exchange on disease prevalence and on sterility levels .
	manualset3
152534	3	408161	13	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Brunham model is an important attempt to model the effects of different assumptions about rates of partner exchange on disease prevalence and on sterility levels .
	manualset3
152535	4	408161	13	NULL	NULL	0	NULL	assumptions	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Brunham model is an important attempt to model the effects of different assumptions about rates of partner exchange on disease prevalence and on sterility levels .
	manualset3
152536	5	408161	13	NULL	NULL	0	NULL	rates of partner exchange	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Brunham model is an important attempt to model the effects of different assumptions about rates of partner exchange on disease prevalence and on sterility levels .
	manualset3
152537	6	408161	13	NULL	NULL	0	NULL	disease prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Brunham model is an important attempt to model the effects of different assumptions about rates of partner exchange on disease prevalence and on sterility levels .
	manualset3
152538	7	408161	13	NULL	NULL	0	NULL	sterility levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Brunham model is an important attempt to model the effects of different assumptions about rates of partner exchange on disease prevalence and on sterility levels .
	manualset3
152539	1	408162	13	NULL	NULL	0	NULL	C-1 portions 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The C-1 portions of their 13C-NMR spectra are typical of the lichen species and indicate differences between the two polysaccharides .
	manualset3
152540	2	408162	13	NULL	NULL	0	NULL	13C-NMR spectra 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The C-1 portions of their 13C-NMR spectra are typical of the lichen species and indicate differences between the two polysaccharides .
	manualset3
152541	3	408162	13	NULL	NULL	0	NULL	lichen species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The C-1 portions of their 13C-NMR spectra are typical of the lichen species and indicate differences between the two polysaccharides .
	manualset3
152542	4	408162	13	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The C-1 portions of their 13C-NMR spectra are typical of the lichen species and indicate differences between the two polysaccharides .
	manualset3
152543	5	408162	13	NULL	NULL	0	NULL	two polysaccharides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The C-1 portions of their 13C-NMR spectra are typical of the lichen species and indicate differences between the two polysaccharides .
	manualset3
152544	1	408163	13	NULL	NULL	0	NULL	C. elegans 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The C. elegans Ce-fkh-1 gene has been cloned on the basis of its sequence similarity to the winged-helix DNA binding domain of the Drosophila fork head and mammalian HNF-3alpha , beta , gamma genes , and mutations in the zygotically active pha-4 gene have been shown to block formation of the pharynx ( and rectum ) at an early stage in embryogenesis .
	manualset3
152545	2	408163	13	NULL	NULL	0	NULL	Ce-fkh-1 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The C. elegans Ce-fkh-1 gene has been cloned on the basis of its sequence similarity to the winged-helix DNA binding domain of the Drosophila fork head and mammalian HNF-3alpha , beta , gamma genes , and mutations in the zygotically active pha-4 gene have been shown to block formation of the pharynx ( and rectum ) at an early stage in embryogenesis .
	manualset3
152546	3	408163	13	NULL	NULL	0	NULL	basis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The C. elegans Ce-fkh-1 gene has been cloned on the basis of its sequence similarity to the winged-helix DNA binding domain of the Drosophila fork head and mammalian HNF-3alpha , beta , gamma genes , and mutations in the zygotically active pha-4 gene have been shown to block formation of the pharynx ( and rectum ) at an early stage in embryogenesis .
	manualset3
152547	4	408163	13	NULL	NULL	0	NULL	sequence similarity	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The C. elegans Ce-fkh-1 gene has been cloned on the basis of its sequence similarity to the winged-helix DNA binding domain of the Drosophila fork head and mammalian HNF-3alpha , beta , gamma genes , and mutations in the zygotically active pha-4 gene have been shown to block formation of the pharynx ( and rectum ) at an early stage in embryogenesis .
	manualset3
152548	5	408163	13	NULL	NULL	0	NULL	winged-helix DNA binding domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The C. elegans Ce-fkh-1 gene has been cloned on the basis of its sequence similarity to the winged-helix DNA binding domain of the Drosophila fork head and mammalian HNF-3alpha , beta , gamma genes , and mutations in the zygotically active pha-4 gene have been shown to block formation of the pharynx ( and rectum ) at an early stage in embryogenesis .
	manualset3
152549	6	408163	13	NULL	NULL	0	NULL	Drosophila fork head	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The C. elegans Ce-fkh-1 gene has been cloned on the basis of its sequence similarity to the winged-helix DNA binding domain of the Drosophila fork head and mammalian HNF-3alpha , beta , gamma genes , and mutations in the zygotically active pha-4 gene have been shown to block formation of the pharynx ( and rectum ) at an early stage in embryogenesis .
	manualset3
152550	7	408163	13	NULL	NULL	0	NULL	mammalian HNF-3alpha gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The C. elegans Ce-fkh-1 gene has been cloned on the basis of its sequence similarity to the winged-helix DNA binding domain of the Drosophila fork head and mammalian HNF-3alpha , beta , gamma genes , and mutations in the zygotically active pha-4 gene have been shown to block formation of the pharynx ( and rectum ) at an early stage in embryogenesis .
	manualset3
152551	8	408163	13	NULL	NULL	0	NULL	mammalian HNF-3beta gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The C. elegans Ce-fkh-1 gene has been cloned on the basis of its sequence similarity to the winged-helix DNA binding domain of the Drosophila fork head and mammalian HNF-3alpha , beta , gamma genes , and mutations in the zygotically active pha-4 gene have been shown to block formation of the pharynx ( and rectum ) at an early stage in embryogenesis .
	manualset3
152552	9	408163	13	NULL	NULL	0	NULL	mammalian HNF-3gamma gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The C. elegans Ce-fkh-1 gene has been cloned on the basis of its sequence similarity to the winged-helix DNA binding domain of the Drosophila fork head and mammalian HNF-3alpha , beta , gamma genes , and mutations in the zygotically active pha-4 gene have been shown to block formation of the pharynx ( and rectum ) at an early stage in embryogenesis .
	manualset3
152553	10	408163	13	NULL	NULL	0	NULL	mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The C. elegans Ce-fkh-1 gene has been cloned on the basis of its sequence similarity to the winged-helix DNA binding domain of the Drosophila fork head and mammalian HNF-3alpha , beta , gamma genes , and mutations in the zygotically active pha-4 gene have been shown to block formation of the pharynx ( and rectum ) at an early stage in embryogenesis .
	manualset3
152554	11	408163	13	NULL	NULL	0	NULL	zygotically active pha-4 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The C. elegans Ce-fkh-1 gene has been cloned on the basis of its sequence similarity to the winged-helix DNA binding domain of the Drosophila fork head and mammalian HNF-3alpha , beta , gamma genes , and mutations in the zygotically active pha-4 gene have been shown to block formation of the pharynx ( and rectum ) at an early stage in embryogenesis .
	manualset3
152555	12	408163	13	NULL	NULL	0	NULL	formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The C. elegans Ce-fkh-1 gene has been cloned on the basis of its sequence similarity to the winged-helix DNA binding domain of the Drosophila fork head and mammalian HNF-3alpha , beta , gamma genes , and mutations in the zygotically active pha-4 gene have been shown to block formation of the pharynx ( and rectum ) at an early stage in embryogenesis .
	manualset3
152556	13	408163	13	NULL	NULL	0	NULL	pharynx 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The C. elegans Ce-fkh-1 gene has been cloned on the basis of its sequence similarity to the winged-helix DNA binding domain of the Drosophila fork head and mammalian HNF-3alpha , beta , gamma genes , and mutations in the zygotically active pha-4 gene have been shown to block formation of the pharynx ( and rectum ) at an early stage in embryogenesis .
	manualset3
152557	14	408163	13	NULL	NULL	0	NULL	rectum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The C. elegans Ce-fkh-1 gene has been cloned on the basis of its sequence similarity to the winged-helix DNA binding domain of the Drosophila fork head and mammalian HNF-3alpha , beta , gamma genes , and mutations in the zygotically active pha-4 gene have been shown to block formation of the pharynx ( and rectum ) at an early stage in embryogenesis .
	manualset3
152558	15	408163	13	NULL	NULL	0	NULL	early stage	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The C. elegans Ce-fkh-1 gene has been cloned on the basis of its sequence similarity to the winged-helix DNA binding domain of the Drosophila fork head and mammalian HNF-3alpha , beta , gamma genes , and mutations in the zygotically active pha-4 gene have been shown to block formation of the pharynx ( and rectum ) at an early stage in embryogenesis .
	manualset3
152559	16	408163	13	NULL	NULL	0	NULL	embryogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The C. elegans Ce-fkh-1 gene has been cloned on the basis of its sequence similarity to the winged-helix DNA binding domain of the Drosophila fork head and mammalian HNF-3alpha , beta , gamma genes , and mutations in the zygotically active pha-4 gene have been shown to block formation of the pharynx ( and rectum ) at an early stage in embryogenesis .
	manualset3
152560	1	408164	13	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomised comparison of this bimonthly high-dose LV/5-FU regimen and the NCCTG-Mayo Clinic regimen ( LV ( 20 mg/m2/day ) followed by 5-FU bolus ( 425 mg/m2/day ) daily x 5 , every 4 weeks ) showed that the bimonthly high-dose LV/5-FU regimen was superior to the NCCTG-Mayo Clinic regimen in response rate and progression-free survival , but showed no difference in overall survival .
	manualset3
152561	2	408164	13	NULL	NULL	0	NULL	high-dose LV/5-FU regimen 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomised comparison of this bimonthly high-dose LV/5-FU regimen and the NCCTG-Mayo Clinic regimen ( LV ( 20 mg/m2/day ) followed by 5-FU bolus ( 425 mg/m2/day ) daily x 5 , every 4 weeks ) showed that the bimonthly high-dose LV/5-FU regimen was superior to the NCCTG-Mayo Clinic regimen in response rate and progression-free survival , but showed no difference in overall survival .
	manualset3
152562	3	408164	13	NULL	NULL	0	NULL	NCCTG-Mayo Clinic regimen 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomised comparison of this bimonthly high-dose LV/5-FU regimen and the NCCTG-Mayo Clinic regimen ( LV ( 20 mg/m2/day ) followed by 5-FU bolus ( 425 mg/m2/day ) daily x 5 , every 4 weeks ) showed that the bimonthly high-dose LV/5-FU regimen was superior to the NCCTG-Mayo Clinic regimen in response rate and progression-free survival , but showed no difference in overall survival .
	manualset3
152563	4	408164	13	NULL	NULL	0	NULL	LV ( 20 mg/m2/day	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomised comparison of this bimonthly high-dose LV/5-FU regimen and the NCCTG-Mayo Clinic regimen ( LV ( 20 mg/m2/day ) followed by 5-FU bolus ( 425 mg/m2/day ) daily x 5 , every 4 weeks ) showed that the bimonthly high-dose LV/5-FU regimen was superior to the NCCTG-Mayo Clinic regimen in response rate and progression-free survival , but showed no difference in overall survival .
	manualset3
152564	5	408164	13	NULL	NULL	0	NULL	5-FU bolus	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomised comparison of this bimonthly high-dose LV/5-FU regimen and the NCCTG-Mayo Clinic regimen ( LV ( 20 mg/m2/day ) followed by 5-FU bolus ( 425 mg/m2/day ) daily x 5 , every 4 weeks ) showed that the bimonthly high-dose LV/5-FU regimen was superior to the NCCTG-Mayo Clinic regimen in response rate and progression-free survival , but showed no difference in overall survival .
	manualset3
152565	6	408164	13	NULL	NULL	0	NULL	425 mg/m2/day	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomised comparison of this bimonthly high-dose LV/5-FU regimen and the NCCTG-Mayo Clinic regimen ( LV ( 20 mg/m2/day ) followed by 5-FU bolus ( 425 mg/m2/day ) daily x 5 , every 4 weeks ) showed that the bimonthly high-dose LV/5-FU regimen was superior to the NCCTG-Mayo Clinic regimen in response rate and progression-free survival , but showed no difference in overall survival .
	manualset3
152566	7	408164	13	NULL	NULL	0	NULL	daily x 5	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomised comparison of this bimonthly high-dose LV/5-FU regimen and the NCCTG-Mayo Clinic regimen ( LV ( 20 mg/m2/day ) followed by 5-FU bolus ( 425 mg/m2/day ) daily x 5 , every 4 weeks ) showed that the bimonthly high-dose LV/5-FU regimen was superior to the NCCTG-Mayo Clinic regimen in response rate and progression-free survival , but showed no difference in overall survival .
	manualset3
152567	8	408164	13	NULL	NULL	0	NULL	4 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomised comparison of this bimonthly high-dose LV/5-FU regimen and the NCCTG-Mayo Clinic regimen ( LV ( 20 mg/m2/day ) followed by 5-FU bolus ( 425 mg/m2/day ) daily x 5 , every 4 weeks ) showed that the bimonthly high-dose LV/5-FU regimen was superior to the NCCTG-Mayo Clinic regimen in response rate and progression-free survival , but showed no difference in overall survival .
	manualset3
152568	9	408164	13	NULL	NULL	0	NULL	 high-dose LV/5-FU regimen	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomised comparison of this bimonthly high-dose LV/5-FU regimen and the NCCTG-Mayo Clinic regimen ( LV ( 20 mg/m2/day ) followed by 5-FU bolus ( 425 mg/m2/day ) daily x 5 , every 4 weeks ) showed that the bimonthly high-dose LV/5-FU regimen was superior to the NCCTG-Mayo Clinic regimen in response rate and progression-free survival , but showed no difference in overall survival .
	manualset3
152569	10	408164	13	NULL	NULL	0	NULL	NCCTG-Mayo Clinic regimen	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomised comparison of this bimonthly high-dose LV/5-FU regimen and the NCCTG-Mayo Clinic regimen ( LV ( 20 mg/m2/day ) followed by 5-FU bolus ( 425 mg/m2/day ) daily x 5 , every 4 weeks ) showed that the bimonthly high-dose LV/5-FU regimen was superior to the NCCTG-Mayo Clinic regimen in response rate and progression-free survival , but showed no difference in overall survival .
	manualset3
152570	11	408164	13	NULL	NULL	0	NULL	response rate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomised comparison of this bimonthly high-dose LV/5-FU regimen and the NCCTG-Mayo Clinic regimen ( LV ( 20 mg/m2/day ) followed by 5-FU bolus ( 425 mg/m2/day ) daily x 5 , every 4 weeks ) showed that the bimonthly high-dose LV/5-FU regimen was superior to the NCCTG-Mayo Clinic regimen in response rate and progression-free survival , but showed no difference in overall survival .
	manualset3
152571	12	408164	13	NULL	NULL	0	NULL	progression-free survival 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomised comparison of this bimonthly high-dose LV/5-FU regimen and the NCCTG-Mayo Clinic regimen ( LV ( 20 mg/m2/day ) followed by 5-FU bolus ( 425 mg/m2/day ) daily x 5 , every 4 weeks ) showed that the bimonthly high-dose LV/5-FU regimen was superior to the NCCTG-Mayo Clinic regimen in response rate and progression-free survival , but showed no difference in overall survival .
	manualset3
152572	13	408164	13	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomised comparison of this bimonthly high-dose LV/5-FU regimen and the NCCTG-Mayo Clinic regimen ( LV ( 20 mg/m2/day ) followed by 5-FU bolus ( 425 mg/m2/day ) daily x 5 , every 4 weeks ) showed that the bimonthly high-dose LV/5-FU regimen was superior to the NCCTG-Mayo Clinic regimen in response rate and progression-free survival , but showed no difference in overall survival .
	manualset3
152573	14	408164	13	NULL	NULL	0	NULL	overall survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomised comparison of this bimonthly high-dose LV/5-FU regimen and the NCCTG-Mayo Clinic regimen ( LV ( 20 mg/m2/day ) followed by 5-FU bolus ( 425 mg/m2/day ) daily x 5 , every 4 weeks ) showed that the bimonthly high-dose LV/5-FU regimen was superior to the NCCTG-Mayo Clinic regimen in response rate and progression-free survival , but showed no difference in overall survival .
	manualset3
152574	1	408165	13	NULL	NULL	0	NULL	C11orf9 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The C11orf9 gene consists of 26 exons spanning 33.1 kb of genomic DNA and is located about 4.3 kb centromeric to FEN1 .
	manualset3
152575	2	408165	13	NULL	NULL	0	NULL	26 exons spanning 33.1 kb of genomic DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The C11orf9 gene consists of 26 exons spanning 33.1 kb of genomic DNA and is located about 4.3 kb centromeric to FEN1 .
	manualset3
152576	3	408165	13	NULL	NULL	0	NULL	 4.3 kb centromeric	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The C11orf9 gene consists of 26 exons spanning 33.1 kb of genomic DNA and is located about 4.3 kb centromeric to FEN1 .
	manualset3
152577	4	408165	13	NULL	NULL	0	NULL	FEN1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The C11orf9 gene consists of 26 exons spanning 33.1 kb of genomic DNA and is located about 4.3 kb centromeric to FEN1 .
	manualset3
152578	1	408166	13	NULL	NULL	0	NULL	C3a molecule 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The C3a molecule is active at submicromolar concentrations and the spasmogenic activities are absolutely dependent on a carboxy-terminal arginyl residue .
	manualset3
152579	2	408166	13	NULL	NULL	NULL	NULL	submicromolar concentrations 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The C3a molecule is active at submicromolar concentrations and the spasmogenic activities are absolutely dependent on a carboxy-terminal arginyl residue .
	manualset3
152580	3	408166	13	NULL	NULL	0	NULL	spasmogenic activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The C3a molecule is active at submicromolar concentrations and the spasmogenic activities are absolutely dependent on a carboxy-terminal arginyl residue .
	manualset3
152581	4	408166	13	NULL	NULL	0	NULL	carboxy-terminal arginyl residue	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The C3a molecule is active at submicromolar concentrations and the spasmogenic activities are absolutely dependent on a carboxy-terminal arginyl residue .
	manualset3
152582	1	408167	13	NULL	NULL	0	NULL	CAC 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The CAC represented a significant regional source of CH4 since the estimated ebullitive fluxes ( 3.5 mg m ( -2 ) h ( -1 ) ) were similar to the CH4 emissions measured above typical flooded freshwater wetlands .
	manualset3
152583	2	408167	13	NULL	NULL	0	NULL	source	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The CAC represented a significant regional source of CH4 since the estimated ebullitive fluxes ( 3.5 mg m ( -2 ) h ( -1 ) ) were similar to the CH4 emissions measured above typical flooded freshwater wetlands .
	manualset3
152584	3	408167	13	NULL	NULL	0	NULL	CH4	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The CAC represented a significant regional source of CH4 since the estimated ebullitive fluxes ( 3.5 mg m ( -2 ) h ( -1 ) ) were similar to the CH4 emissions measured above typical flooded freshwater wetlands .
	manualset3
152585	4	408167	13	NULL	NULL	0	NULL	ebullitive fluxes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The CAC represented a significant regional source of CH4 since the estimated ebullitive fluxes ( 3.5 mg m ( -2 ) h ( -1 ) ) were similar to the CH4 emissions measured above typical flooded freshwater wetlands .
	manualset3
152586	5	408167	13	NULL	NULL	0	NULL	3.5 mg m ( -2 ) h ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The CAC represented a significant regional source of CH4 since the estimated ebullitive fluxes ( 3.5 mg m ( -2 ) h ( -1 ) ) were similar to the CH4 emissions measured above typical flooded freshwater wetlands .
	manualset3
152587	6	408167	13	NULL	NULL	0	NULL	CH4 emissions 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The CAC represented a significant regional source of CH4 since the estimated ebullitive fluxes ( 3.5 mg m ( -2 ) h ( -1 ) ) were similar to the CH4 emissions measured above typical flooded freshwater wetlands .
	manualset3
152588	7	408167	13	NULL	NULL	0	NULL	freshwater wetlands	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The CAC represented a significant regional source of CH4 since the estimated ebullitive fluxes ( 3.5 mg m ( -2 ) h ( -1 ) ) were similar to the CH4 emissions measured above typical flooded freshwater wetlands .
	manualset3
152589	1	408168	13	NULL	NULL	NULL	NULL	CAH group	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The CAH group , showed a 32.5 % of positiveness with a maximum levels of 25pg aflatoxin lysine/mg albumin while 20 % of HBsAg positive carriers showed levels of un 12.3 pg aflatoxin lysine/mg albumin and 15 % of the control group 5pg AF lysine/mg albumin .
	manualset3
152590	2	408168	13	NULL	NULL	0	NULL	32.5 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The CAH group , showed a 32.5 % of positiveness with a maximum levels of 25pg aflatoxin lysine/mg albumin while 20 % of HBsAg positive carriers showed levels of un 12.3 pg aflatoxin lysine/mg albumin and 15 % of the control group 5pg AF lysine/mg albumin .
	manualset3
152591	3	408168	13	NULL	NULL	0	NULL	positiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The CAH group , showed a 32.5 % of positiveness with a maximum levels of 25pg aflatoxin lysine/mg albumin while 20 % of HBsAg positive carriers showed levels of un 12.3 pg aflatoxin lysine/mg albumin and 15 % of the control group 5pg AF lysine/mg albumin .
	manualset3
152592	4	408168	13	NULL	NULL	0	NULL	levels of 25pg aflatoxin lysine/mg albumin	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The CAH group , showed a 32.5 % of positiveness with a maximum levels of 25pg aflatoxin lysine/mg albumin while 20 % of HBsAg positive carriers showed levels of un 12.3 pg aflatoxin lysine/mg albumin and 15 % of the control group 5pg AF lysine/mg albumin .
	manualset3
152593	5	408168	13	NULL	NULL	0	NULL	20 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The CAH group , showed a 32.5 % of positiveness with a maximum levels of 25pg aflatoxin lysine/mg albumin while 20 % of HBsAg positive carriers showed levels of un 12.3 pg aflatoxin lysine/mg albumin and 15 % of the control group 5pg AF lysine/mg albumin .
	manualset3
152594	6	408168	13	NULL	NULL	0	NULL	HBsAg positive carriers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The CAH group , showed a 32.5 % of positiveness with a maximum levels of 25pg aflatoxin lysine/mg albumin while 20 % of HBsAg positive carriers showed levels of un 12.3 pg aflatoxin lysine/mg albumin and 15 % of the control group 5pg AF lysine/mg albumin .
	manualset3
152595	7	408168	13	NULL	NULL	0	NULL	levels of un 12.3 pg aflatoxin lysine/mg albumin	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The CAH group , showed a 32.5 % of positiveness with a maximum levels of 25pg aflatoxin lysine/mg albumin while 20 % of HBsAg positive carriers showed levels of un 12.3 pg aflatoxin lysine/mg albumin and 15 % of the control group 5pg AF lysine/mg albumin .
	manualset3
152596	8	408168	13	NULL	NULL	0	NULL	15 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The CAH group , showed a 32.5 % of positiveness with a maximum levels of 25pg aflatoxin lysine/mg albumin while 20 % of HBsAg positive carriers showed levels of un 12.3 pg aflatoxin lysine/mg albumin and 15 % of the control group 5pg AF lysine/mg albumin .
	manualset3
152597	9	408168	13	NULL	NULL	0	NULL	control group 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The CAH group , showed a 32.5 % of positiveness with a maximum levels of 25pg aflatoxin lysine/mg albumin while 20 % of HBsAg positive carriers showed levels of un 12.3 pg aflatoxin lysine/mg albumin and 15 % of the control group 5pg AF lysine/mg albumin .
	manualset3
152598	10	408168	13	NULL	NULL	0	NULL	5pg AF lysine/mg albumin	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The CAH group , showed a 32.5 % of positiveness with a maximum levels of 25pg aflatoxin lysine/mg albumin while 20 % of HBsAg positive carriers showed levels of un 12.3 pg aflatoxin lysine/mg albumin and 15 % of the control group 5pg AF lysine/mg albumin .
	manualset3
152599	1	408169	13	NULL	NULL	0	NULL	CASE-J extension	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The CASE-J extension , which covered a 3-year extension of follow-up from the original trial , corroborated the results of the CASE-J trial .
	manualset3
152600	2	408169	13	NULL	NULL	0	NULL	3-year extension	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The CASE-J extension , which covered a 3-year extension of follow-up from the original trial , corroborated the results of the CASE-J trial .
	manualset3
152601	3	408169	13	NULL	NULL	0	NULL	follow-up 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The CASE-J extension , which covered a 3-year extension of follow-up from the original trial , corroborated the results of the CASE-J trial .
	manualset3
152602	4	408169	13	NULL	NULL	0	NULL	original trial	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The CASE-J extension , which covered a 3-year extension of follow-up from the original trial , corroborated the results of the CASE-J trial .
	manualset3
152603	5	408169	13	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The CASE-J extension , which covered a 3-year extension of follow-up from the original trial , corroborated the results of the CASE-J trial .
	manualset3
152604	6	408169	13	NULL	NULL	0	NULL	CASE-J trial	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The CASE-J extension , which covered a 3-year extension of follow-up from the original trial , corroborated the results of the CASE-J trial .
	manualset3
152605	1	408170	13	NULL	NULL	0	NULL	CAT gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The CAT gene was expressed in all tissues examined , demonstrating that the hEF1 alpha promoter was active in a wide range of mouse cells .
	manualset3
152606	2	408170	13	NULL	NULL	0	NULL	 tissues 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The CAT gene was expressed in all tissues examined , demonstrating that the hEF1 alpha promoter was active in a wide range of mouse cells .
	manualset3
152607	3	408170	13	NULL	NULL	0	NULL	 hEF1 alpha promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The CAT gene was expressed in all tissues examined , demonstrating that the hEF1 alpha promoter was active in a wide range of mouse cells .
	manualset3
152608	4	408170	13	NULL	NULL	0	NULL	range	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The CAT gene was expressed in all tissues examined , demonstrating that the hEF1 alpha promoter was active in a wide range of mouse cells .
	manualset3
152609	5	408170	13	NULL	NULL	0	NULL	 mouse cells	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The CAT gene was expressed in all tissues examined , demonstrating that the hEF1 alpha promoter was active in a wide range of mouse cells .
	manualset3
152610	1	408171	13	NULL	NULL	0	NULL	CAT	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The CAT was developed in 2009 and implemented in 2010 .
	manualset3
152611	2	408171	13	NULL	NULL	0	NULL	2009 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The CAT was developed in 2009 and implemented in 2010 .
	manualset3
152612	3	408171	13	NULL	NULL	0	NULL	 2010 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The CAT was developed in 2009 and implemented in 2010 .
	manualset3
152613	1	408172	13	NULL	NULL	0	NULL	CB cytokine	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The CB cytokine and chemokine levels from children of 20 allergic and 36 non-allergic women were determined by a multiplexed Luminex assay and ELISA .
	manualset3
152614	2	408172	13	NULL	NULL	0	NULL	chemokine	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The CB cytokine and chemokine levels from children of 20 allergic and 36 non-allergic women were determined by a multiplexed Luminex assay and ELISA .
	manualset3
152615	3	408172	13	NULL	NULL	0	NULL	levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The CB cytokine and chemokine levels from children of 20 allergic and 36 non-allergic women were determined by a multiplexed Luminex assay and ELISA .
	manualset3
152616	4	408172	13	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The CB cytokine and chemokine levels from children of 20 allergic and 36 non-allergic women were determined by a multiplexed Luminex assay and ELISA .
	manualset3
152617	5	408172	13	NULL	NULL	0	NULL	20 allergic women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The CB cytokine and chemokine levels from children of 20 allergic and 36 non-allergic women were determined by a multiplexed Luminex assay and ELISA .
	manualset3
152618	6	408172	13	NULL	NULL	0	NULL	36 non-allergic women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The CB cytokine and chemokine levels from children of 20 allergic and 36 non-allergic women were determined by a multiplexed Luminex assay and ELISA .
	manualset3
152619	7	408172	13	NULL	NULL	0	NULL	 multiplexed Luminex assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The CB cytokine and chemokine levels from children of 20 allergic and 36 non-allergic women were determined by a multiplexed Luminex assay and ELISA .
	manualset3
152620	8	408172	13	NULL	NULL	0	NULL	ELISA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The CB cytokine and chemokine levels from children of 20 allergic and 36 non-allergic women were determined by a multiplexed Luminex assay and ELISA .
	manualset3
152621	1	408173	13	NULL	NULL	0	NULL	CBFs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The CBFs on the contralateral side were lower than those in the BOT group , but the vasoreactivity was similar .
	manualset3
152622	2	408173	13	NULL	NULL	0	NULL	contralateral side	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The CBFs on the contralateral side were lower than those in the BOT group , but the vasoreactivity was similar .
	manualset3
152623	3	408173	13	NULL	NULL	0	NULL	BOT group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The CBFs on the contralateral side were lower than those in the BOT group , but the vasoreactivity was similar .
	manualset3
152624	4	408173	13	NULL	NULL	0	NULL	vasoreactivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The CBFs on the contralateral side were lower than those in the BOT group , but the vasoreactivity was similar .
	manualset3
152625	1	408174	13	NULL	NULL	0	NULL	CDA activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The CDA activity of DY-52 was maximal ( 20 U/mg ) on the 3rd day of culture in the same medium .
	manualset3
152626	2	408174	13	NULL	NULL	0	NULL	DY-52	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The CDA activity of DY-52 was maximal ( 20 U/mg ) on the 3rd day of culture in the same medium .
	manualset3
152627	3	408174	13	NULL	NULL	0	NULL	20 U/mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The CDA activity of DY-52 was maximal ( 20 U/mg ) on the 3rd day of culture in the same medium .
	manualset3
152628	4	408174	13	NULL	NULL	0	NULL	3rd day 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The CDA activity of DY-52 was maximal ( 20 U/mg ) on the 3rd day of culture in the same medium .
	manualset3
152629	5	408174	13	NULL	NULL	0	NULL	culture	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The CDA activity of DY-52 was maximal ( 20 U/mg ) on the 3rd day of culture in the same medium .
	manualset3
152630	6	408174	13	NULL	NULL	NULL	NULL	medium	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The CDA activity of DY-52 was maximal ( 20 U/mg ) on the 3rd day of culture in the same medium .
	manualset3
152631	1	408175	13	NULL	NULL	0	NULL	 pilot trial 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomised controlled pilot trial to evaluate and optimize the use of anti-platelet agents in the perioperative management in patients undergoing general and abdominal surgery -- the APAP trial ( ISRCTN45810007 ) .
	manualset3
152632	2	408175	13	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomised controlled pilot trial to evaluate and optimize the use of anti-platelet agents in the perioperative management in patients undergoing general and abdominal surgery -- the APAP trial ( ISRCTN45810007 ) .
	manualset3
152633	3	408175	13	NULL	NULL	0	NULL	anti-platelet agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomised controlled pilot trial to evaluate and optimize the use of anti-platelet agents in the perioperative management in patients undergoing general and abdominal surgery -- the APAP trial ( ISRCTN45810007 ) .
	manualset3
152634	4	408175	13	NULL	NULL	0	NULL	perioperative management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomised controlled pilot trial to evaluate and optimize the use of anti-platelet agents in the perioperative management in patients undergoing general and abdominal surgery -- the APAP trial ( ISRCTN45810007 ) .
	manualset3
152635	5	408175	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomised controlled pilot trial to evaluate and optimize the use of anti-platelet agents in the perioperative management in patients undergoing general and abdominal surgery -- the APAP trial ( ISRCTN45810007 ) .
	manualset3
152636	6	408175	13	NULL	NULL	0	NULL	 abdominal surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomised controlled pilot trial to evaluate and optimize the use of anti-platelet agents in the perioperative management in patients undergoing general and abdominal surgery -- the APAP trial ( ISRCTN45810007 ) .
	manualset3
152637	7	408175	13	NULL	NULL	0	NULL	APAP trial ( ISRCTN45810007 )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomised controlled pilot trial to evaluate and optimize the use of anti-platelet agents in the perioperative management in patients undergoing general and abdominal surgery -- the APAP trial ( ISRCTN45810007 ) .
	manualset3
152638	1	408176	13	NULL	NULL	0	NULL	CDC WONDER-based information system	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The CDC WONDER-based information system crosslinks the objectives , data sets , and assessments and provides 5-10 pages of information about each .
	manualset3
152639	2	408176	13	NULL	NULL	0	NULL	objectives	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The CDC WONDER-based information system crosslinks the objectives , data sets , and assessments and provides 5-10 pages of information about each .
	manualset3
152640	3	408176	13	NULL	NULL	0	NULL	data sets	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The CDC WONDER-based information system crosslinks the objectives , data sets , and assessments and provides 5-10 pages of information about each .
	manualset3
152641	4	408176	13	NULL	NULL	0	NULL	assessments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The CDC WONDER-based information system crosslinks the objectives , data sets , and assessments and provides 5-10 pages of information about each .
	manualset3
152642	5	408176	13	NULL	NULL	0	NULL	 5-10 pages	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The CDC WONDER-based information system crosslinks the objectives , data sets , and assessments and provides 5-10 pages of information about each .
	manualset3
152643	6	408176	13	NULL	NULL	0	NULL	information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The CDC WONDER-based information system crosslinks the objectives , data sets , and assessments and provides 5-10 pages of information about each .
	manualset3
152644	1	408177	13	NULL	NULL	0	NULL	CF tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The CF tissue exhibited an adherent layer of mucus similar to the mucus plaques reported in the distal airways of human CF patients .
	manualset3
152645	2	408177	13	NULL	NULL	0	NULL	adherent layer of mucus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The CF tissue exhibited an adherent layer of mucus similar to the mucus plaques reported in the distal airways of human CF patients .
	manualset3
152646	3	408177	13	NULL	NULL	0	NULL	mucus plaques	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The CF tissue exhibited an adherent layer of mucus similar to the mucus plaques reported in the distal airways of human CF patients .
	manualset3
152647	4	408177	13	NULL	NULL	0	NULL	distal airways 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The CF tissue exhibited an adherent layer of mucus similar to the mucus plaques reported in the distal airways of human CF patients .
	manualset3
152648	5	408177	13	NULL	NULL	0	NULL	 human CF patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The CF tissue exhibited an adherent layer of mucus similar to the mucus plaques reported in the distal airways of human CF patients .
	manualset3
152650	1	408178	13	NULL	NULL	0	NULL	CHESS 19F MRI technique provides	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The CHESS 19F MRI technique provides useful physiological and biochemical data on the biodistribution of the antineoplastic drug 5-FU and on the different catabolic activities of the tissues .
	manualset3
152651	2	408178	13	NULL	NULL	0	NULL	physiological data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The CHESS 19F MRI technique provides useful physiological and biochemical data on the biodistribution of the antineoplastic drug 5-FU and on the different catabolic activities of the tissues .
	manualset3
152652	3	408178	13	NULL	NULL	0	NULL	biochemical data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The CHESS 19F MRI technique provides useful physiological and biochemical data on the biodistribution of the antineoplastic drug 5-FU and on the different catabolic activities of the tissues .
	manualset3
152653	4	408178	13	NULL	NULL	NULL	NULL	 biodistribution 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The CHESS 19F MRI technique provides useful physiological and biochemical data on the biodistribution of the antineoplastic drug 5-FU and on the different catabolic activities of the tissues .
	manualset3
152654	5	408178	13	NULL	NULL	0	NULL	antineoplastic drug 5-FU	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The CHESS 19F MRI technique provides useful physiological and biochemical data on the biodistribution of the antineoplastic drug 5-FU and on the different catabolic activities of the tissues .
	manualset3
152655	6	408178	13	NULL	NULL	0	NULL	catabolic activities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The CHESS 19F MRI technique provides useful physiological and biochemical data on the biodistribution of the antineoplastic drug 5-FU and on the different catabolic activities of the tissues .
	manualset3
152656	7	408178	13	NULL	NULL	0	NULL	tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The CHESS 19F MRI technique provides useful physiological and biochemical data on the biodistribution of the antineoplastic drug 5-FU and on the different catabolic activities of the tissues .
	manualset3
152657	1	408179	13	NULL	NULL	0	NULL	CIDR device 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The CIDR device is comparable to the MAP sponge for estrus synchrony during the breeding season , and reasonable fertility can be achieved without the use of PMSG .
	manualset3
152658	2	408179	13	NULL	NULL	0	NULL	MAP sponge	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The CIDR device is comparable to the MAP sponge for estrus synchrony during the breeding season , and reasonable fertility can be achieved without the use of PMSG .
	manualset3
152659	3	408179	13	NULL	NULL	0	NULL	estrus synchrony	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The CIDR device is comparable to the MAP sponge for estrus synchrony during the breeding season , and reasonable fertility can be achieved without the use of PMSG .
	manualset3
152660	4	408179	13	NULL	NULL	0	NULL	breeding season	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The CIDR device is comparable to the MAP sponge for estrus synchrony during the breeding season , and reasonable fertility can be achieved without the use of PMSG .
	manualset3
152661	5	408179	13	NULL	NULL	0	NULL	reasonable fertility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The CIDR device is comparable to the MAP sponge for estrus synchrony during the breeding season , and reasonable fertility can be achieved without the use of PMSG .
	manualset3
152662	6	408179	13	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The CIDR device is comparable to the MAP sponge for estrus synchrony during the breeding season , and reasonable fertility can be achieved without the use of PMSG .
	manualset3
152663	7	408179	13	NULL	NULL	0	NULL	PMSG	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The CIDR device is comparable to the MAP sponge for estrus synchrony during the breeding season , and reasonable fertility can be achieved without the use of PMSG .
	manualset3
152709	1	408180	13	NULL	NULL	0	NULL	CK2 gene products	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The CK2 and ' catalytic gene products have overlapping biochemical activity , but in vivo , their functions are very different .
	manualset3
152710	2	408180	13	NULL	NULL	0	NULL	catalytic gene products 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The CK2 and ' catalytic gene products have overlapping biochemical activity , but in vivo , their functions are very different .
	manualset3
152711	3	408180	13	NULL	NULL	0	NULL	biochemical activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The CK2 and ' catalytic gene products have overlapping biochemical activity , but in vivo , their functions are very different .
	manualset3
152712	4	408180	13	NULL	NULL	0	NULL	functions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The CK2 and ' catalytic gene products have overlapping biochemical activity , but in vivo , their functions are very different .
	manualset3
152714	1	408181	13	NULL	NULL	0	NULL	CL species	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The CL species distribution in various organs appeared to be in agreement with prior reports .
	manualset3
152715	2	408181	13	NULL	NULL	0	NULL	 distribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The CL species distribution in various organs appeared to be in agreement with prior reports .
	manualset3
152716	3	408181	13	NULL	NULL	0	NULL	organs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The CL species distribution in various organs appeared to be in agreement with prior reports .
	manualset3
152717	4	408181	13	NULL	NULL	0	NULL	agreement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The CL species distribution in various organs appeared to be in agreement with prior reports .
	manualset3
152718	5	408181	13	NULL	NULL	0	NULL	prior reports	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The CL species distribution in various organs appeared to be in agreement with prior reports .
	manualset3
152719	1	408182	13	NULL	NULL	0	NULL	CMV promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The CMV promoter initially expressed 10 - to 100-fold higher levels of EGFP compared to EF1alpha or PGK , respectively , at increasing MOI , although a significant decline in transgene expression was observed posttransduction and with advancing passage ( P & lt ; 0.01 ) , whereas a significant increase in the level of expression was observed over time with the EF1alpha promoter .
	manualset3
152720	2	408182	13	NULL	NULL	NULL	NULL	10 - to 100-fold higher levels	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The CMV promoter initially expressed 10 - to 100-fold higher levels of EGFP compared to EF1alpha or PGK , respectively , at increasing MOI , although a significant decline in transgene expression was observed posttransduction and with advancing passage ( P & lt ; 0.01 ) , whereas a significant increase in the level of expression was observed over time with the EF1alpha promoter .
	manualset3
152721	3	408182	13	NULL	NULL	NULL	NULL	EGFP 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The CMV promoter initially expressed 10 - to 100-fold higher levels of EGFP compared to EF1alpha or PGK , respectively , at increasing MOI , although a significant decline in transgene expression was observed posttransduction and with advancing passage ( P & lt ; 0.01 ) , whereas a significant increase in the level of expression was observed over time with the EF1alpha promoter .
	manualset3
152722	4	408182	13	NULL	NULL	NULL	NULL	EF1alpha	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The CMV promoter initially expressed 10 - to 100-fold higher levels of EGFP compared to EF1alpha or PGK , respectively , at increasing MOI , although a significant decline in transgene expression was observed posttransduction and with advancing passage ( P & lt ; 0.01 ) , whereas a significant increase in the level of expression was observed over time with the EF1alpha promoter .
	manualset3
152723	5	408182	13	NULL	NULL	0	NULL	PGK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The CMV promoter initially expressed 10 - to 100-fold higher levels of EGFP compared to EF1alpha or PGK , respectively , at increasing MOI , although a significant decline in transgene expression was observed posttransduction and with advancing passage ( P & lt ; 0.01 ) , whereas a significant increase in the level of expression was observed over time with the EF1alpha promoter .
	manualset3
152724	6	408182	13	NULL	NULL	0	NULL	MOI	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The CMV promoter initially expressed 10 - to 100-fold higher levels of EGFP compared to EF1alpha or PGK , respectively , at increasing MOI , although a significant decline in transgene expression was observed posttransduction and with advancing passage ( P & lt ; 0.01 ) , whereas a significant increase in the level of expression was observed over time with the EF1alpha promoter .
	manualset3
152725	7	408182	13	NULL	NULL	0	NULL	decline 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The CMV promoter initially expressed 10 - to 100-fold higher levels of EGFP compared to EF1alpha or PGK , respectively , at increasing MOI , although a significant decline in transgene expression was observed posttransduction and with advancing passage ( P & lt ; 0.01 ) , whereas a significant increase in the level of expression was observed over time with the EF1alpha promoter .
	manualset3
152726	8	408182	13	NULL	NULL	0	NULL	transgene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The CMV promoter initially expressed 10 - to 100-fold higher levels of EGFP compared to EF1alpha or PGK , respectively , at increasing MOI , although a significant decline in transgene expression was observed posttransduction and with advancing passage ( P & lt ; 0.01 ) , whereas a significant increase in the level of expression was observed over time with the EF1alpha promoter .
	manualset3
152727	9	408182	13	NULL	NULL	0	NULL	posttransduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The CMV promoter initially expressed 10 - to 100-fold higher levels of EGFP compared to EF1alpha or PGK , respectively , at increasing MOI , although a significant decline in transgene expression was observed posttransduction and with advancing passage ( P & lt ; 0.01 ) , whereas a significant increase in the level of expression was observed over time with the EF1alpha promoter .
	manualset3
152728	10	408182	13	NULL	NULL	0	NULL	passage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The CMV promoter initially expressed 10 - to 100-fold higher levels of EGFP compared to EF1alpha or PGK , respectively , at increasing MOI , although a significant decline in transgene expression was observed posttransduction and with advancing passage ( P & lt ; 0.01 ) , whereas a significant increase in the level of expression was observed over time with the EF1alpha promoter .
	manualset3
152729	11	408182	13	NULL	NULL	0	NULL	P & lt ; 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The CMV promoter initially expressed 10 - to 100-fold higher levels of EGFP compared to EF1alpha or PGK , respectively , at increasing MOI , although a significant decline in transgene expression was observed posttransduction and with advancing passage ( P & lt ; 0.01 ) , whereas a significant increase in the level of expression was observed over time with the EF1alpha promoter .
	manualset3
152730	12	408182	13	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The CMV promoter initially expressed 10 - to 100-fold higher levels of EGFP compared to EF1alpha or PGK , respectively , at increasing MOI , although a significant decline in transgene expression was observed posttransduction and with advancing passage ( P & lt ; 0.01 ) , whereas a significant increase in the level of expression was observed over time with the EF1alpha promoter .
	manualset3
152731	13	408182	13	NULL	NULL	0	NULL	level 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The CMV promoter initially expressed 10 - to 100-fold higher levels of EGFP compared to EF1alpha or PGK , respectively , at increasing MOI , although a significant decline in transgene expression was observed posttransduction and with advancing passage ( P & lt ; 0.01 ) , whereas a significant increase in the level of expression was observed over time with the EF1alpha promoter .
	manualset3
152732	14	408182	13	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The CMV promoter initially expressed 10 - to 100-fold higher levels of EGFP compared to EF1alpha or PGK , respectively , at increasing MOI , although a significant decline in transgene expression was observed posttransduction and with advancing passage ( P & lt ; 0.01 ) , whereas a significant increase in the level of expression was observed over time with the EF1alpha promoter .
	manualset3
152733	15	408182	13	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The CMV promoter initially expressed 10 - to 100-fold higher levels of EGFP compared to EF1alpha or PGK , respectively , at increasing MOI , although a significant decline in transgene expression was observed posttransduction and with advancing passage ( P & lt ; 0.01 ) , whereas a significant increase in the level of expression was observed over time with the EF1alpha promoter .
	manualset3
152734	16	408182	13	NULL	NULL	0	NULL	EF1alpha promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The CMV promoter initially expressed 10 - to 100-fold higher levels of EGFP compared to EF1alpha or PGK , respectively , at increasing MOI , although a significant decline in transgene expression was observed posttransduction and with advancing passage ( P & lt ; 0.01 ) , whereas a significant increase in the level of expression was observed over time with the EF1alpha promoter .
	manualset3
152735	1	408183	13	NULL	NULL	0	NULL	COOH terminal region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The COOH terminal region of the alpha-amylase of pTUB4 was encoded in pUB110 .
	manualset3
152736	2	408183	13	NULL	NULL	0	NULL	alpha-amylase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The COOH terminal region of the alpha-amylase of pTUB4 was encoded in pUB110 .
	manualset3
152737	3	408183	13	NULL	NULL	0	NULL	pTUB4	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The COOH terminal region of the alpha-amylase of pTUB4 was encoded in pUB110 .
	manualset3
152738	4	408183	13	NULL	NULL	0	NULL	 pUB110	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The COOH terminal region of the alpha-amylase of pTUB4 was encoded in pUB110 .
	manualset3
152739	1	408184	13	NULL	NULL	0	NULL	CR extract BNO 1055	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The CR extract BNO 1055 was devoid of any effect on ERalpha gene expression .
	manualset3
152740	2	408184	13	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The CR extract BNO 1055 was devoid of any effect on ERalpha gene expression .
	manualset3
152741	3	408184	13	NULL	NULL	0	NULL	ERalpha gene expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The CR extract BNO 1055 was devoid of any effect on ERalpha gene expression .
	manualset3
152742	1	408185	13	NULL	NULL	0	NULL	CSF accumulator	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The CSF accumulator : its role in the central nervous system and implications for advancing hydrocephalus shunt technology .
	manualset3
152743	2	408185	13	NULL	NULL	0	NULL	role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The CSF accumulator : its role in the central nervous system and implications for advancing hydrocephalus shunt technology .
	manualset3
152744	3	408185	13	NULL	NULL	0	NULL	central nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The CSF accumulator : its role in the central nervous system and implications for advancing hydrocephalus shunt technology .
	manualset3
152745	4	408185	13	NULL	NULL	0	NULL	implications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The CSF accumulator : its role in the central nervous system and implications for advancing hydrocephalus shunt technology .
	manualset3
152746	5	408185	13	NULL	NULL	0	NULL	 hydrocephalus shunt technology 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The CSF accumulator : its role in the central nervous system and implications for advancing hydrocephalus shunt technology .
	manualset3
152747	1	408186	13	NULL	NULL	0	NULL	CTLp frequencies	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The CTLp frequencies against controls , sharing no HLA antigens with the blood transfusion donor , were only slightly increased ( up to 5 times ) in 7 patients and decreased in 3 .
	manualset3
152748	2	408186	13	NULL	NULL	0	NULL	controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The CTLp frequencies against controls , sharing no HLA antigens with the blood transfusion donor , were only slightly increased ( up to 5 times ) in 7 patients and decreased in 3 .
	manualset3
152749	3	408186	13	NULL	NULL	0	NULL	HLA antigens	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The CTLp frequencies against controls , sharing no HLA antigens with the blood transfusion donor , were only slightly increased ( up to 5 times ) in 7 patients and decreased in 3 .
	manualset3
152750	4	408186	13	NULL	NULL	0	NULL	blood transfusion donor	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The CTLp frequencies against controls , sharing no HLA antigens with the blood transfusion donor , were only slightly increased ( up to 5 times ) in 7 patients and decreased in 3 .
	manualset3
152751	5	408186	13	NULL	NULL	0	NULL	5 times 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The CTLp frequencies against controls , sharing no HLA antigens with the blood transfusion donor , were only slightly increased ( up to 5 times ) in 7 patients and decreased in 3 .
	manualset3
152752	6	408186	13	NULL	NULL	0	NULL	7 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The CTLp frequencies against controls , sharing no HLA antigens with the blood transfusion donor , were only slightly increased ( up to 5 times ) in 7 patients and decreased in 3 .
	manualset3
152753	7	408186	13	NULL	NULL	0	NULL	3	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The CTLp frequencies against controls , sharing no HLA antigens with the blood transfusion donor , were only slightly increased ( up to 5 times ) in 7 patients and decreased in 3 .
	manualset3
152754	1	408187	13	NULL	NULL	0	NULL	 CTP 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The CTP is a good sampling method for studies of Demodex prevalence .
	manualset3
152755	2	408187	13	NULL	NULL	0	NULL	sampling method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The CTP is a good sampling method for studies of Demodex prevalence .
	manualset3
152756	3	408187	13	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The CTP is a good sampling method for studies of Demodex prevalence .
	manualset3
152757	4	408187	13	NULL	NULL	0	NULL	Demodex prevalence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The CTP is a good sampling method for studies of Demodex prevalence .
	manualset3
152758	1	408188	13	NULL	NULL	0	NULL	CV	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The CV was about 14 % for all elutriated fractions .
	manualset3
152759	2	408188	13	NULL	NULL	0	NULL	 14 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The CV was about 14 % for all elutriated fractions .
	manualset3
152760	3	408188	13	NULL	NULL	NULL	NULL	fractions	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The CV was about 14 % for all elutriated fractions .
	manualset3
152761	1	408189	13	NULL	NULL	0	NULL	C/EBP-homologous transcription factor CHOP ( GADD153 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The C/EBP-homologous transcription factor CHOP ( GADD153 ) is inducible by growth inhibition or DNA damage , and has been shown to be oncogenically activated by the specific ( 12 ; 16 ) translocation in human myxoid liposarcoma .
	manualset3
152762	2	408189	13	NULL	NULL	0	NULL	growth inhibition 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The C/EBP-homologous transcription factor CHOP ( GADD153 ) is inducible by growth inhibition or DNA damage , and has been shown to be oncogenically activated by the specific ( 12 ; 16 ) translocation in human myxoid liposarcoma .
	manualset3
152763	3	408189	13	NULL	NULL	0	NULL	DNA damage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The C/EBP-homologous transcription factor CHOP ( GADD153 ) is inducible by growth inhibition or DNA damage , and has been shown to be oncogenically activated by the specific ( 12 ; 16 ) translocation in human myxoid liposarcoma .
	manualset3
152764	4	408189	13	NULL	NULL	0	NULL	12 ; 16 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The C/EBP-homologous transcription factor CHOP ( GADD153 ) is inducible by growth inhibition or DNA damage , and has been shown to be oncogenically activated by the specific ( 12 ; 16 ) translocation in human myxoid liposarcoma .
	manualset3
152765	5	408189	13	NULL	NULL	0	NULL	translocation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The C/EBP-homologous transcription factor CHOP ( GADD153 ) is inducible by growth inhibition or DNA damage , and has been shown to be oncogenically activated by the specific ( 12 ; 16 ) translocation in human myxoid liposarcoma .
	manualset3
152766	6	408189	13	NULL	NULL	0	NULL	 human myxoid liposarcoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The C/EBP-homologous transcription factor CHOP ( GADD153 ) is inducible by growth inhibition or DNA damage , and has been shown to be oncogenically activated by the specific ( 12 ; 16 ) translocation in human myxoid liposarcoma .
	manualset3
152767	1	408190	13	NULL	NULL	0	NULL	Ca2 + - dependent ATPase activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Ca2 + - dependent ATPase activity can be reversibly inhibited by ethanol , which changes the divalent cation dependency from Ca2 + to Mg2 + .
	manualset3
152768	2	408190	13	NULL	NULL	0	NULL	ethanol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The Ca2 + - dependent ATPase activity can be reversibly inhibited by ethanol , which changes the divalent cation dependency from Ca2 + to Mg2 + .
	manualset3
152769	3	408190	13	NULL	NULL	0	NULL	divalent cation dependency	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Ca2 + - dependent ATPase activity can be reversibly inhibited by ethanol , which changes the divalent cation dependency from Ca2 + to Mg2 + .
	manualset3
152770	4	408190	13	NULL	NULL	0	NULL	Ca2 + 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The Ca2 + - dependent ATPase activity can be reversibly inhibited by ethanol , which changes the divalent cation dependency from Ca2 + to Mg2 + .
	manualset3
152771	5	408190	13	NULL	NULL	0	NULL	Mg2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The Ca2 + - dependent ATPase activity can be reversibly inhibited by ethanol , which changes the divalent cation dependency from Ca2 + to Mg2 + .
	manualset3
152772	1	408191	13	NULL	NULL	0	NULL	Can82853-01 genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The Can82853-01 genome was 7 , 322 nucleotides ( nt ) in length and had 96.4 % , 77.7 % , and 77.5 % nt identity with the A308/99 ( HPeV-3 ) , HPeV-1 , and HPeV-2 reference strains , respectively .
	manualset3
152773	2	408191	13	NULL	NULL	0	NULL	7 , 322 nucleotides ( nt ) 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The Can82853-01 genome was 7 , 322 nucleotides ( nt ) in length and had 96.4 % , 77.7 % , and 77.5 % nt identity with the A308/99 ( HPeV-3 ) , HPeV-1 , and HPeV-2 reference strains , respectively .
	manualset3
152774	3	408191	13	NULL	NULL	0	NULL	length	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Can82853-01 genome was 7 , 322 nucleotides ( nt ) in length and had 96.4 % , 77.7 % , and 77.5 % nt identity with the A308/99 ( HPeV-3 ) , HPeV-1 , and HPeV-2 reference strains , respectively .
	manualset3
152775	4	408191	13	NULL	NULL	0	NULL	96.4 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Can82853-01 genome was 7 , 322 nucleotides ( nt ) in length and had 96.4 % , 77.7 % , and 77.5 % nt identity with the A308/99 ( HPeV-3 ) , HPeV-1 , and HPeV-2 reference strains , respectively .
	manualset3
152776	5	408191	13	NULL	NULL	0	NULL	77.7 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Can82853-01 genome was 7 , 322 nucleotides ( nt ) in length and had 96.4 % , 77.7 % , and 77.5 % nt identity with the A308/99 ( HPeV-3 ) , HPeV-1 , and HPeV-2 reference strains , respectively .
	manualset3
152777	6	408191	13	NULL	NULL	0	NULL	77.5 % nt identity	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Can82853-01 genome was 7 , 322 nucleotides ( nt ) in length and had 96.4 % , 77.7 % , and 77.5 % nt identity with the A308/99 ( HPeV-3 ) , HPeV-1 , and HPeV-2 reference strains , respectively .
	manualset3
152778	7	408191	13	NULL	NULL	0	NULL	A308/99 ( HPeV-3 ) strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The Can82853-01 genome was 7 , 322 nucleotides ( nt ) in length and had 96.4 % , 77.7 % , and 77.5 % nt identity with the A308/99 ( HPeV-3 ) , HPeV-1 , and HPeV-2 reference strains , respectively .
	manualset3
152779	8	408191	13	NULL	NULL	0	NULL	HPeV-1strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The Can82853-01 genome was 7 , 322 nucleotides ( nt ) in length and had 96.4 % , 77.7 % , and 77.5 % nt identity with the A308/99 ( HPeV-3 ) , HPeV-1 , and HPeV-2 reference strains , respectively .
	manualset3
152780	9	408191	13	NULL	NULL	0	NULL	HPeV-2 reference strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The Can82853-01 genome was 7 , 322 nucleotides ( nt ) in length and had 96.4 % , 77.7 % , and 77.5 % nt identity with the A308/99 ( HPeV-3 ) , HPeV-1 , and HPeV-2 reference strains , respectively .
	manualset3
152781	1	408192	13	NULL	NULL	NULL	NULL	Centers for Disease Control and Prevention ( CDC )	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The Centers for Disease Control and Prevention ( CDC ) recommends STI screening as part of routine HIV care .
	manualset3
152783	3	408192	13	NULL	NULL	0	NULL	STI screening	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The Centers for Disease Control and Prevention ( CDC ) recommends STI screening as part of routine HIV care .
	manualset3
152784	4	408192	13	NULL	NULL	0	NULL	routine HIV care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The Centers for Disease Control and Prevention ( CDC ) recommends STI screening as part of routine HIV care .
	manualset3
152785	1	408193	13	NULL	NULL	0	NULL	double-blinded study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized , double-blinded study evaluating the immunogenicity , safety and consistency of production of a combined diphtheria-tetanus-pertussis-Haemophilus influenzae type b vaccine entirely produced in Brazil by Bio-Manguinhos and Instituto Butantan ( DTP/Hib-BM ) was undertaken .
	manualset3
152786	2	408193	13	NULL	NULL	0	NULL	immunogenicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized , double-blinded study evaluating the immunogenicity , safety and consistency of production of a combined diphtheria-tetanus-pertussis-Haemophilus influenzae type b vaccine entirely produced in Brazil by Bio-Manguinhos and Instituto Butantan ( DTP/Hib-BM ) was undertaken .
	manualset3
152787	3	408193	13	NULL	NULL	0	NULL	safety	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized , double-blinded study evaluating the immunogenicity , safety and consistency of production of a combined diphtheria-tetanus-pertussis-Haemophilus influenzae type b vaccine entirely produced in Brazil by Bio-Manguinhos and Instituto Butantan ( DTP/Hib-BM ) was undertaken .
	manualset3
152788	4	408193	13	NULL	NULL	0	NULL	consistency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized , double-blinded study evaluating the immunogenicity , safety and consistency of production of a combined diphtheria-tetanus-pertussis-Haemophilus influenzae type b vaccine entirely produced in Brazil by Bio-Manguinhos and Instituto Butantan ( DTP/Hib-BM ) was undertaken .
	manualset3
152789	5	408193	13	NULL	NULL	0	NULL	production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized , double-blinded study evaluating the immunogenicity , safety and consistency of production of a combined diphtheria-tetanus-pertussis-Haemophilus influenzae type b vaccine entirely produced in Brazil by Bio-Manguinhos and Instituto Butantan ( DTP/Hib-BM ) was undertaken .
	manualset3
152790	6	408193	13	NULL	NULL	0	NULL	diphtheria-tetanus-pertussis-Haemophilus influenzae type b vaccine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized , double-blinded study evaluating the immunogenicity , safety and consistency of production of a combined diphtheria-tetanus-pertussis-Haemophilus influenzae type b vaccine entirely produced in Brazil by Bio-Manguinhos and Instituto Butantan ( DTP/Hib-BM ) was undertaken .
	manualset3
152791	7	408193	13	NULL	NULL	0	NULL	Brazil 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized , double-blinded study evaluating the immunogenicity , safety and consistency of production of a combined diphtheria-tetanus-pertussis-Haemophilus influenzae type b vaccine entirely produced in Brazil by Bio-Manguinhos and Instituto Butantan ( DTP/Hib-BM ) was undertaken .
	manualset3
152792	8	408193	13	NULL	NULL	0	NULL	Bio-Manguinhos	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized , double-blinded study evaluating the immunogenicity , safety and consistency of production of a combined diphtheria-tetanus-pertussis-Haemophilus influenzae type b vaccine entirely produced in Brazil by Bio-Manguinhos and Instituto Butantan ( DTP/Hib-BM ) was undertaken .
	manualset3
152793	9	408193	13	NULL	NULL	0	NULL	Instituto Butantan ( DTP/Hib-BM ) 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized , double-blinded study evaluating the immunogenicity , safety and consistency of production of a combined diphtheria-tetanus-pertussis-Haemophilus influenzae type b vaccine entirely produced in Brazil by Bio-Manguinhos and Instituto Butantan ( DTP/Hib-BM ) was undertaken .
	manualset3
152794	1	408194	13	NULL	NULL	0	NULL	Cln3-knockout ( Cln3 - / - ) mouse model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The Cln3-knockout ( Cln3 - / - ) mouse model of the disease exhibits many characteristic pathological features of the human disorder .
	manualset3
152795	2	408194	13	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The Cln3-knockout ( Cln3 - / - ) mouse model of the disease exhibits many characteristic pathological features of the human disorder .
	manualset3
152796	3	408194	13	NULL	NULL	0	NULL	pathological features 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Cln3-knockout ( Cln3 - / - ) mouse model of the disease exhibits many characteristic pathological features of the human disorder .
	manualset3
152797	4	408194	13	NULL	NULL	0	NULL	human disorder 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The Cln3-knockout ( Cln3 - / - ) mouse model of the disease exhibits many characteristic pathological features of the human disorder .
	manualset3
152798	1	408195	13	NULL	NULL	0	NULL	Concerns About Recurrence Scale ( CARS )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Concerns About Recurrence Scale ( CARS ) systematically assesses the extent and nature of women 's fears about the possibility of breast cancer recurrence .
	manualset3
152799	2	408195	13	NULL	NULL	0	NULL	extent 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Concerns About Recurrence Scale ( CARS ) systematically assesses the extent and nature of women 's fears about the possibility of breast cancer recurrence .
	manualset3
152800	3	408195	13	NULL	NULL	0	NULL	nature	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Concerns About Recurrence Scale ( CARS ) systematically assesses the extent and nature of women 's fears about the possibility of breast cancer recurrence .
	manualset3
152801	4	408195	13	NULL	NULL	0	NULL	women 's fears	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Concerns About Recurrence Scale ( CARS ) systematically assesses the extent and nature of women 's fears about the possibility of breast cancer recurrence .
	manualset3
152802	5	408195	13	NULL	NULL	0	NULL	possibility 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Concerns About Recurrence Scale ( CARS ) systematically assesses the extent and nature of women 's fears about the possibility of breast cancer recurrence .
	manualset3
152803	6	408195	13	NULL	NULL	0	NULL	breast cancer recurrence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Concerns About Recurrence Scale ( CARS ) systematically assesses the extent and nature of women 's fears about the possibility of breast cancer recurrence .
	manualset3
152804	1	408196	13	NULL	NULL	NULL	NULL	Consortium for Radiologic Imaging Studies of Polycystic Kidney Disease ( CRISP ) 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The Consortium for Radiologic Imaging Studies of Polycystic Kidney Disease ( CRISP ) was created to develop imaging techniques and analyses to evaluate progression .
	manualset3
152805	2	408196	13	NULL	NULL	NULL	NULL	imaging techniques	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The Consortium for Radiologic Imaging Studies of Polycystic Kidney Disease ( CRISP ) was created to develop imaging techniques and analyses to evaluate progression .
	manualset3
152806	3	408196	13	NULL	NULL	0	NULL	analyses	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The Consortium for Radiologic Imaging Studies of Polycystic Kidney Disease ( CRISP ) was created to develop imaging techniques and analyses to evaluate progression .
	manualset3
152807	4	408196	13	NULL	NULL	0	NULL	progression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Consortium for Radiologic Imaging Studies of Polycystic Kidney Disease ( CRISP ) was created to develop imaging techniques and analyses to evaluate progression .
	manualset3
152808	1	408197	13	NULL	NULL	0	NULL	Cox regression test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Cox regression test displayed significant values for age , histologic diagnosis , and PCNA determinations when considered in tandem .
	manualset3
152809	2	408197	13	NULL	NULL	0	NULL	values for age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Cox regression test displayed significant values for age , histologic diagnosis , and PCNA determinations when considered in tandem .
	manualset3
152810	3	408197	13	NULL	NULL	0	NULL	histologic diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The Cox regression test displayed significant values for age , histologic diagnosis , and PCNA determinations when considered in tandem .
	manualset3
152811	4	408197	13	NULL	NULL	0	NULL	PCNA determinations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Cox regression test displayed significant values for age , histologic diagnosis , and PCNA determinations when considered in tandem .
	manualset3
152812	5	408197	13	NULL	NULL	0	NULL	 tandem	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Cox regression test displayed significant values for age , histologic diagnosis , and PCNA determinations when considered in tandem .
	manualset3
152813	1	408198	13	NULL	NULL	0	NULL	Coxeter group	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Coxeter group of reflections of this billiard is discrete and is the Weyl group of the hyperbolic Kac-Moody algebra E10 ( for type II ) or BE10 ( for type I or heterotic ) , which are both arithmetic .
	manualset3
152814	2	408198	13	NULL	NULL	0	NULL	reflections	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Coxeter group of reflections of this billiard is discrete and is the Weyl group of the hyperbolic Kac-Moody algebra E10 ( for type II ) or BE10 ( for type I or heterotic ) , which are both arithmetic .
	manualset3
152815	3	408198	13	NULL	NULL	0	NULL	billiard 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The Coxeter group of reflections of this billiard is discrete and is the Weyl group of the hyperbolic Kac-Moody algebra E10 ( for type II ) or BE10 ( for type I or heterotic ) , which are both arithmetic .
	manualset3
152816	4	408198	13	NULL	NULL	0	NULL	Weyl group 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The Coxeter group of reflections of this billiard is discrete and is the Weyl group of the hyperbolic Kac-Moody algebra E10 ( for type II ) or BE10 ( for type I or heterotic ) , which are both arithmetic .
	manualset3
152817	5	408198	13	NULL	NULL	0	NULL	hyperbolic Kac-Moody algebra E10 ( for type II ) 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The Coxeter group of reflections of this billiard is discrete and is the Weyl group of the hyperbolic Kac-Moody algebra E10 ( for type II ) or BE10 ( for type I or heterotic ) , which are both arithmetic .
	manualset3
152818	6	408198	13	NULL	NULL	0	NULL	BE10 ( for type I or heterotic ) 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The Coxeter group of reflections of this billiard is discrete and is the Weyl group of the hyperbolic Kac-Moody algebra E10 ( for type II ) or BE10 ( for type I or heterotic ) , which are both arithmetic .
	manualset3
152822	1	408199	13	NULL	NULL	0	NULL	Characteristics 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Characteristics of cytotoxic t-lymphocytes eluted from allogenic target cells ) .
	manualset3
152823	2	408199	13	NULL	NULL	0	NULL	cytotoxic t-lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	( Characteristics of cytotoxic t-lymphocytes eluted from allogenic target cells ) .
	manualset3
152824	3	408199	13	NULL	NULL	0	NULL	allogenic target cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	( Characteristics of cytotoxic t-lymphocytes eluted from allogenic target cells ) .
	manualset3
152830	1	408200	13	NULL	NULL	0	NULL	Cs ( + ) cation sites	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The Cs ( + ) cation sites are fully occupied , ordered , and located in the cavities of the framework .
	manualset3
152834	2	408200	13	NULL	NULL	0	NULL	cavities	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The Cs ( + ) cation sites are fully occupied , ordered , and located in the cavities of the framework .
	manualset3
152840	3	408200	13	NULL	NULL	0	NULL	framework	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The Cs ( + ) cation sites are fully occupied , ordered , and located in the cavities of the framework .
	manualset3
152845	1	408201	13	NULL	NULL	0	NULL	D-dimer concentration 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The D-dimer concentration was assessed in patients ' plasma with the use of immunoturbidometry .
	manualset3
152847	2	408201	13	NULL	NULL	0	NULL	patients ' plasma 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The D-dimer concentration was assessed in patients ' plasma with the use of immunoturbidometry .
	manualset3
152849	3	408201	13	NULL	NULL	0	NULL	immunoturbidometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The D-dimer concentration was assessed in patients ' plasma with the use of immunoturbidometry .
	manualset3
152851	4	408201	13	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The D-dimer concentration was assessed in patients ' plasma with the use of immunoturbidometry .
	manualset3
152854	1	408202	13	NULL	NULL	0	NULL	D2-agonist bromocriptine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The D2-agonist bromocriptine acts on these projection cells and loss of these through 3-NPA administration resulted in a significant decrease of locomotor activity and a substantial attenuation of the BOLD-response in the striatum .
	manualset3
152856	2	408202	13	NULL	NULL	0	NULL	acts 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The D2-agonist bromocriptine acts on these projection cells and loss of these through 3-NPA administration resulted in a significant decrease of locomotor activity and a substantial attenuation of the BOLD-response in the striatum .
	manualset3
152857	3	408202	13	NULL	NULL	0	NULL	projection cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The D2-agonist bromocriptine acts on these projection cells and loss of these through 3-NPA administration resulted in a significant decrease of locomotor activity and a substantial attenuation of the BOLD-response in the striatum .
	manualset3
152858	4	408202	13	NULL	NULL	0	NULL	loss 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The D2-agonist bromocriptine acts on these projection cells and loss of these through 3-NPA administration resulted in a significant decrease of locomotor activity and a substantial attenuation of the BOLD-response in the striatum .
	manualset3
152862	5	408202	13	NULL	NULL	0	NULL	 3-NPA administration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The D2-agonist bromocriptine acts on these projection cells and loss of these through 3-NPA administration resulted in a significant decrease of locomotor activity and a substantial attenuation of the BOLD-response in the striatum .
	manualset3
152863	6	408202	13	NULL	NULL	0	NULL	decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The D2-agonist bromocriptine acts on these projection cells and loss of these through 3-NPA administration resulted in a significant decrease of locomotor activity and a substantial attenuation of the BOLD-response in the striatum .
	manualset3
152864	7	408202	13	NULL	NULL	0	NULL	locomotor activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The D2-agonist bromocriptine acts on these projection cells and loss of these through 3-NPA administration resulted in a significant decrease of locomotor activity and a substantial attenuation of the BOLD-response in the striatum .
	manualset3
152866	8	408202	13	NULL	NULL	0	NULL	attenuation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The D2-agonist bromocriptine acts on these projection cells and loss of these through 3-NPA administration resulted in a significant decrease of locomotor activity and a substantial attenuation of the BOLD-response in the striatum .
	manualset3
152869	9	408202	13	NULL	NULL	0	NULL	BOLD-response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The D2-agonist bromocriptine acts on these projection cells and loss of these through 3-NPA administration resulted in a significant decrease of locomotor activity and a substantial attenuation of the BOLD-response in the striatum .
	manualset3
152870	10	408202	13	NULL	NULL	0	NULL	striatum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The D2-agonist bromocriptine acts on these projection cells and loss of these through 3-NPA administration resulted in a significant decrease of locomotor activity and a substantial attenuation of the BOLD-response in the striatum .
	manualset3
152873	1	408203	13	NULL	NULL	0	NULL	D5 receptor plasmid	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The D5 receptor plasmid ( hD5R/pcDNA3 .1 ) and reporter gene plasmid ( 4 x CRE/TK/Luci / pGL3 ) were co-transfected into HEK293 cell line .
	manualset3
152874	2	408203	13	NULL	NULL	0	NULL	hD5R/pcDNA3 .1	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The D5 receptor plasmid ( hD5R/pcDNA3 .1 ) and reporter gene plasmid ( 4 x CRE/TK/Luci / pGL3 ) were co-transfected into HEK293 cell line .
	manualset3
152875	3	408203	13	NULL	NULL	0	NULL	reporter gene plasmid	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The D5 receptor plasmid ( hD5R/pcDNA3 .1 ) and reporter gene plasmid ( 4 x CRE/TK/Luci / pGL3 ) were co-transfected into HEK293 cell line .
	manualset3
152876	4	408203	13	NULL	NULL	0	NULL	4 x CRE/TK/Luci / pGL3	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The D5 receptor plasmid ( hD5R/pcDNA3 .1 ) and reporter gene plasmid ( 4 x CRE/TK/Luci / pGL3 ) were co-transfected into HEK293 cell line .
	manualset3
152878	5	408203	13	NULL	NULL	0	NULL	HEK293 cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The D5 receptor plasmid ( hD5R/pcDNA3 .1 ) and reporter gene plasmid ( 4 x CRE/TK/Luci / pGL3 ) were co-transfected into HEK293 cell line .
	manualset3
152882	1	408204	13	NULL	NULL	0	NULL	 DMF ratio	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The DMF ratio increased with age in all patients with OI type I and was higher among the patients with OI type III and DI .
	manualset3
152883	2	408204	13	NULL	NULL	0	NULL	age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The DMF ratio increased with age in all patients with OI type I and was higher among the patients with OI type III and DI .
	manualset3
152884	3	408204	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The DMF ratio increased with age in all patients with OI type I and was higher among the patients with OI type III and DI .
	manualset3
152885	4	408204	13	NULL	NULL	0	NULL	OI type I 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The DMF ratio increased with age in all patients with OI type I and was higher among the patients with OI type III and DI .
	manualset3
152887	5	408204	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The DMF ratio increased with age in all patients with OI type I and was higher among the patients with OI type III and DI .
	manualset3
152888	6	408204	13	NULL	NULL	0	NULL	OI type III 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The DMF ratio increased with age in all patients with OI type I and was higher among the patients with OI type III and DI .
	manualset3
152890	7	408204	13	NULL	NULL	0	NULL	OI type DI	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The DMF ratio increased with age in all patients with OI type I and was higher among the patients with OI type III and DI .
	manualset3
152918	1	408205	13	NULL	NULL	0	NULL	DNA-binding protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA-binding protein , RdgC , is associated with recombination and replication fork repair in Escherichia coli and with the virulence-associated , pilin antigenic variation mediated by RecA and other recombination proteins in Neisseria species .
	manualset3
152919	2	408205	13	NULL	NULL	0	NULL	RdgC 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA-binding protein , RdgC , is associated with recombination and replication fork repair in Escherichia coli and with the virulence-associated , pilin antigenic variation mediated by RecA and other recombination proteins in Neisseria species .
	manualset3
152920	3	408205	13	NULL	NULL	0	NULL	recombination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA-binding protein , RdgC , is associated with recombination and replication fork repair in Escherichia coli and with the virulence-associated , pilin antigenic variation mediated by RecA and other recombination proteins in Neisseria species .
	manualset3
152921	4	408205	13	NULL	NULL	0	NULL	replication fork repair	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA-binding protein , RdgC , is associated with recombination and replication fork repair in Escherichia coli and with the virulence-associated , pilin antigenic variation mediated by RecA and other recombination proteins in Neisseria species .
	manualset3
152923	5	408205	13	NULL	NULL	0	NULL	Escherichia coli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA-binding protein , RdgC , is associated with recombination and replication fork repair in Escherichia coli and with the virulence-associated , pilin antigenic variation mediated by RecA and other recombination proteins in Neisseria species .
	manualset3
152925	6	408205	13	NULL	NULL	0	NULL	pilin antigenic variation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA-binding protein , RdgC , is associated with recombination and replication fork repair in Escherichia coli and with the virulence-associated , pilin antigenic variation mediated by RecA and other recombination proteins in Neisseria species .
	manualset3
152926	7	408205	13	NULL	NULL	0	NULL	RecA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA-binding protein , RdgC , is associated with recombination and replication fork repair in Escherichia coli and with the virulence-associated , pilin antigenic variation mediated by RecA and other recombination proteins in Neisseria species .
	manualset3
152928	8	408205	13	NULL	NULL	0	NULL	recombination proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA-binding protein , RdgC , is associated with recombination and replication fork repair in Escherichia coli and with the virulence-associated , pilin antigenic variation mediated by RecA and other recombination proteins in Neisseria species .
	manualset3
152930	9	408205	13	NULL	NULL	0	NULL	Neisseria species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA-binding protein , RdgC , is associated with recombination and replication fork repair in Escherichia coli and with the virulence-associated , pilin antigenic variation mediated by RecA and other recombination proteins in Neisseria species .
	manualset3
152933	1	408206	13	NULL	NULL	0	NULL	DNA G+C content	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA G+C content was 42.0 mol % .
	manualset3
152934	2	408206	13	NULL	NULL	0	NULL	 42.0 mol %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA G+C content was 42.0 mol % .
	manualset3
152940	1	408207	13	NULL	NULL	0	NULL	DNA analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA analysis of the Notch 3 gene identified a novel missense mutation Cys174Phe in this patient .
	manualset3
152941	2	408207	13	NULL	NULL	0	NULL	Notch 3 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA analysis of the Notch 3 gene identified a novel missense mutation Cys174Phe in this patient .
	manualset3
152943	3	408207	13	NULL	NULL	0	NULL	missense mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA analysis of the Notch 3 gene identified a novel missense mutation Cys174Phe in this patient .
	manualset3
152944	4	408207	13	NULL	NULL	0	NULL	Cys174Phe	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA analysis of the Notch 3 gene identified a novel missense mutation Cys174Phe in this patient .
	manualset3
152945	5	408207	13	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA analysis of the Notch 3 gene identified a novel missense mutation Cys174Phe in this patient .
	manualset3
152947	1	408208	13	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA is formulated to a mannosilated particle to target antigen-presenting cells and to protect the DNA from intracellular degradation .
	manualset3
152948	2	408208	13	NULL	NULL	NULL	NULL	particle 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The DNA is formulated to a mannosilated particle to target antigen-presenting cells and to protect the DNA from intracellular degradation .
	manualset3
152949	4	408208	13	NULL	NULL	NULL	NULL	antigen-presenting cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The DNA is formulated to a mannosilated particle to target antigen-presenting cells and to protect the DNA from intracellular degradation .
	manualset3
152950	5	408208	13	NULL	NULL	NULL	NULL	DNA	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The DNA is formulated to a mannosilated particle to target antigen-presenting cells and to protect the DNA from intracellular degradation .
	manualset3
152951	6	408208	13	NULL	NULL	NULL	NULL	intracellular degradation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The DNA is formulated to a mannosilated particle to target antigen-presenting cells and to protect the DNA from intracellular degradation .
	manualset3
152952	3	408208	13	NULL	NULL	NULL	NULL	target	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The DNA is formulated to a mannosilated particle to target antigen-presenting cells and to protect the DNA from intracellular degradation .
	manualset3
152953	1	408209	13	NULL	NULL	0	NULL	DNA repair protein O6-methylguanine-DNA methyltransferase ( MGMT )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA repair protein O6-methylguanine-DNA methyltransferase ( MGMT ) is responsible for the repair of these potentially cytotoxic lesions and may underlie tumor resistance to CENUs .
	manualset3
152954	2	408209	13	NULL	NULL	0	NULL	repair	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA repair protein O6-methylguanine-DNA methyltransferase ( MGMT ) is responsible for the repair of these potentially cytotoxic lesions and may underlie tumor resistance to CENUs .
	manualset3
152955	3	408209	13	NULL	NULL	0	NULL	cytotoxic lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA repair protein O6-methylguanine-DNA methyltransferase ( MGMT ) is responsible for the repair of these potentially cytotoxic lesions and may underlie tumor resistance to CENUs .
	manualset3
152956	4	408209	13	NULL	NULL	0	NULL	tumor resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA repair protein O6-methylguanine-DNA methyltransferase ( MGMT ) is responsible for the repair of these potentially cytotoxic lesions and may underlie tumor resistance to CENUs .
	manualset3
152957	5	408209	13	NULL	NULL	0	NULL	CENUs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA repair protein O6-methylguanine-DNA methyltransferase ( MGMT ) is responsible for the repair of these potentially cytotoxic lesions and may underlie tumor resistance to CENUs .
	manualset3
152958	1	408210	13	NULL	NULL	0	NULL	DNA status	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA status of spermatozoa has been determined using the metachromatic properties of acridine orange ( AO ) .
	manualset3
152959	2	408210	13	NULL	NULL	0	NULL	spermatozoa	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA status of spermatozoa has been determined using the metachromatic properties of acridine orange ( AO ) .
	manualset3
152960	3	408210	13	NULL	NULL	0	NULL	metachromatic properties	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA status of spermatozoa has been determined using the metachromatic properties of acridine orange ( AO ) .
	manualset3
152961	4	408210	13	NULL	NULL	0	NULL	acridine orange ( AO ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The DNA status of spermatozoa has been determined using the metachromatic properties of acridine orange ( AO ) .
	manualset3
152962	1	408211	13	NULL	NULL	0	NULL	DVD	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The DVD was evaluated in a randomized controlled trial in which 108 men with hemophilia completed measures of readiness to self-manage pain ( Pain Stages of Change Questionnaire ) before and 6 months after receiving the DVD plus information booklet ( n = 57 ) or just the booklet ( n = 51 ) .
	manualset3
152963	2	408211	13	NULL	NULL	NULL	NULL	randomized controlled trial	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The DVD was evaluated in a randomized controlled trial in which 108 men with hemophilia completed measures of readiness to self-manage pain ( Pain Stages of Change Questionnaire ) before and 6 months after receiving the DVD plus information booklet ( n = 57 ) or just the booklet ( n = 51 ) .
	manualset3
152964	3	408211	13	NULL	NULL	0	NULL	108 men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The DVD was evaluated in a randomized controlled trial in which 108 men with hemophilia completed measures of readiness to self-manage pain ( Pain Stages of Change Questionnaire ) before and 6 months after receiving the DVD plus information booklet ( n = 57 ) or just the booklet ( n = 51 ) .
	manualset3
152965	4	408211	13	NULL	NULL	0	NULL	hemophilia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The DVD was evaluated in a randomized controlled trial in which 108 men with hemophilia completed measures of readiness to self-manage pain ( Pain Stages of Change Questionnaire ) before and 6 months after receiving the DVD plus information booklet ( n = 57 ) or just the booklet ( n = 51 ) .
	manualset3
152966	5	408211	13	NULL	NULL	0	NULL	measures of readiness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The DVD was evaluated in a randomized controlled trial in which 108 men with hemophilia completed measures of readiness to self-manage pain ( Pain Stages of Change Questionnaire ) before and 6 months after receiving the DVD plus information booklet ( n = 57 ) or just the booklet ( n = 51 ) .
	manualset3
152967	6	408211	13	NULL	NULL	0	NULL	 pain 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The DVD was evaluated in a randomized controlled trial in which 108 men with hemophilia completed measures of readiness to self-manage pain ( Pain Stages of Change Questionnaire ) before and 6 months after receiving the DVD plus information booklet ( n = 57 ) or just the booklet ( n = 51 ) .
	manualset3
152968	7	408211	13	NULL	NULL	NULL	NULL	Pain Stages of Change Questionnaire	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The DVD was evaluated in a randomized controlled trial in which 108 men with hemophilia completed measures of readiness to self-manage pain ( Pain Stages of Change Questionnaire ) before and 6 months after receiving the DVD plus information booklet ( n = 57 ) or just the booklet ( n = 51 ) .
	manualset3
152970	9	408211	13	NULL	NULL	0	NULL	 6 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The DVD was evaluated in a randomized controlled trial in which 108 men with hemophilia completed measures of readiness to self-manage pain ( Pain Stages of Change Questionnaire ) before and 6 months after receiving the DVD plus information booklet ( n = 57 ) or just the booklet ( n = 51 ) .
	manualset3
152971	10	408211	13	NULL	NULL	0	NULL	DVD 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The DVD was evaluated in a randomized controlled trial in which 108 men with hemophilia completed measures of readiness to self-manage pain ( Pain Stages of Change Questionnaire ) before and 6 months after receiving the DVD plus information booklet ( n = 57 ) or just the booklet ( n = 51 ) .
	manualset3
152972	11	408211	13	NULL	NULL	0	NULL	 information booklet 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The DVD was evaluated in a randomized controlled trial in which 108 men with hemophilia completed measures of readiness to self-manage pain ( Pain Stages of Change Questionnaire ) before and 6 months after receiving the DVD plus information booklet ( n = 57 ) or just the booklet ( n = 51 ) .
	manualset3
152973	12	408211	13	NULL	NULL	0	NULL	n = 57	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The DVD was evaluated in a randomized controlled trial in which 108 men with hemophilia completed measures of readiness to self-manage pain ( Pain Stages of Change Questionnaire ) before and 6 months after receiving the DVD plus information booklet ( n = 57 ) or just the booklet ( n = 51 ) .
	manualset3
152974	13	408211	13	NULL	NULL	0	NULL	booklet	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The DVD was evaluated in a randomized controlled trial in which 108 men with hemophilia completed measures of readiness to self-manage pain ( Pain Stages of Change Questionnaire ) before and 6 months after receiving the DVD plus information booklet ( n = 57 ) or just the booklet ( n = 51 ) .
	manualset3
152975	14	408211	13	NULL	NULL	0	NULL	n = 51	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The DVD was evaluated in a randomized controlled trial in which 108 men with hemophilia completed measures of readiness to self-manage pain ( Pain Stages of Change Questionnaire ) before and 6 months after receiving the DVD plus information booklet ( n = 57 ) or just the booklet ( n = 51 ) .
	manualset3
152976	1	408212	13	NULL	NULL	0	NULL	Department	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The Department of Health 's End of Life Care Strategy provided the opportunity to develop effective care , regardless of the setting .
	manualset3
152977	2	408212	13	NULL	NULL	0	NULL	Health 's End of Life Care Strategy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The Department of Health 's End of Life Care Strategy provided the opportunity to develop effective care , regardless of the setting .
	manualset3
152978	3	408212	13	NULL	NULL	0	NULL	 opportunity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Department of Health 's End of Life Care Strategy provided the opportunity to develop effective care , regardless of the setting .
	manualset3
152979	4	408212	13	NULL	NULL	0	NULL	effective care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The Department of Health 's End of Life Care Strategy provided the opportunity to develop effective care , regardless of the setting .
	manualset3
152980	5	408212	13	NULL	NULL	0	NULL	setting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Department of Health 's End of Life Care Strategy provided the opportunity to develop effective care , regardless of the setting .
	manualset3
152981	1	408213	13	NULL	NULL	0	NULL	E : I ratio 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The E : I ratio was lowered but it was still slightly larger outside than during attacks .
	manualset3
152982	2	408213	13	NULL	NULL	0	NULL	attacks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The E : I ratio was lowered but it was still slightly larger outside than during attacks .
	manualset3
152983	1	408214	13	NULL	NULL	0	NULL	E protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The E protein of satellite phage P4 acts as an anti-repressor by binding to the C protein of helper phage P2 .
	manualset3
152984	2	408214	13	NULL	NULL	0	NULL	 satellite phage P4 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The E protein of satellite phage P4 acts as an anti-repressor by binding to the C protein of helper phage P2 .
	manualset3
152986	4	408214	13	NULL	NULL	0	NULL	anti-repressor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The E protein of satellite phage P4 acts as an anti-repressor by binding to the C protein of helper phage P2 .
	manualset3
152987	5	408214	13	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The E protein of satellite phage P4 acts as an anti-repressor by binding to the C protein of helper phage P2 .
	manualset3
152988	6	408214	13	NULL	NULL	0	NULL	C protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The E protein of satellite phage P4 acts as an anti-repressor by binding to the C protein of helper phage P2 .
	manualset3
152989	7	408214	13	NULL	NULL	0	NULL	helper phage P2	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The E protein of satellite phage P4 acts as an anti-repressor by binding to the C protein of helper phage P2 .
	manualset3
152990	1	408215	13	NULL	NULL	0	NULL	EBD Champion program	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The EBD Champion program is developing a network of oral health care workers who will disseminate information about the application of an evidence-based approach to dental care and will serve as resources and mentors to their colleagues .
	manualset3
152991	2	408215	13	NULL	NULL	0	NULL	network of oral health care workers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The EBD Champion program is developing a network of oral health care workers who will disseminate information about the application of an evidence-based approach to dental care and will serve as resources and mentors to their colleagues .
	manualset3
152992	3	408215	13	NULL	NULL	0	NULL	information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The EBD Champion program is developing a network of oral health care workers who will disseminate information about the application of an evidence-based approach to dental care and will serve as resources and mentors to their colleagues .
	manualset3
152993	4	408215	13	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The EBD Champion program is developing a network of oral health care workers who will disseminate information about the application of an evidence-based approach to dental care and will serve as resources and mentors to their colleagues .
	manualset3
152994	5	408215	13	NULL	NULL	0	NULL	evidence-based approach	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The EBD Champion program is developing a network of oral health care workers who will disseminate information about the application of an evidence-based approach to dental care and will serve as resources and mentors to their colleagues .
	manualset3
152995	6	408215	13	NULL	NULL	0	NULL	dental care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The EBD Champion program is developing a network of oral health care workers who will disseminate information about the application of an evidence-based approach to dental care and will serve as resources and mentors to their colleagues .
	manualset3
152996	7	408215	13	NULL	NULL	0	NULL	resources	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The EBD Champion program is developing a network of oral health care workers who will disseminate information about the application of an evidence-based approach to dental care and will serve as resources and mentors to their colleagues .
	manualset3
152997	8	408215	13	NULL	NULL	0	NULL	mentors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The EBD Champion program is developing a network of oral health care workers who will disseminate information about the application of an evidence-based approach to dental care and will serve as resources and mentors to their colleagues .
	manualset3
152998	9	408215	13	NULL	NULL	0	NULL	colleagues	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The EBD Champion program is developing a network of oral health care workers who will disseminate information about the application of an evidence-based approach to dental care and will serve as resources and mentors to their colleagues .
	manualset3
152999	1	408216	13	NULL	NULL	0	NULL	EC50 values 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The EC50 values for the increase in ( Ca2 + ) i induced by PAF and ET-18-OCH3 were 5 x 10 ( -11 ) and 2.5 x 10 ( -7 ) M , respectively .
	manualset3
153000	2	408216	13	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The EC50 values for the increase in ( Ca2 + ) i induced by PAF and ET-18-OCH3 were 5 x 10 ( -11 ) and 2.5 x 10 ( -7 ) M , respectively .
	manualset3
153001	3	408216	13	NULL	NULL	0	NULL	( Ca2 + ) i	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The EC50 values for the increase in ( Ca2 + ) i induced by PAF and ET-18-OCH3 were 5 x 10 ( -11 ) and 2.5 x 10 ( -7 ) M , respectively .
	manualset3
153002	4	408216	13	NULL	NULL	0	NULL	PAF	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The EC50 values for the increase in ( Ca2 + ) i induced by PAF and ET-18-OCH3 were 5 x 10 ( -11 ) and 2.5 x 10 ( -7 ) M , respectively .
	manualset3
153003	5	408216	13	NULL	NULL	0	NULL	ET-18-OCH3	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The EC50 values for the increase in ( Ca2 + ) i induced by PAF and ET-18-OCH3 were 5 x 10 ( -11 ) and 2.5 x 10 ( -7 ) M , respectively .
	manualset3
153004	6	408216	13	NULL	NULL	0	NULL	5 x 10 ( -11 ) M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The EC50 values for the increase in ( Ca2 + ) i induced by PAF and ET-18-OCH3 were 5 x 10 ( -11 ) and 2.5 x 10 ( -7 ) M , respectively .
	manualset3
153005	7	408216	13	NULL	NULL	0	NULL	2.5 x 10 ( -7 ) M 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The EC50 values for the increase in ( Ca2 + ) i induced by PAF and ET-18-OCH3 were 5 x 10 ( -11 ) and 2.5 x 10 ( -7 ) M , respectively .
	manualset3
153006	1	408217	13	NULL	NULL	0	NULL	surgical adjuvant trial 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized surgical adjuvant trial in 242 evaluable patients with T1-3a , N0-1 , and M0 breast cancer was initiated 4 years ago .
	manualset3
153007	2	408217	13	NULL	NULL	0	NULL	242 evaluable patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized surgical adjuvant trial in 242 evaluable patients with T1-3a , N0-1 , and M0 breast cancer was initiated 4 years ago .
	manualset3
153008	3	408217	13	NULL	NULL	0	NULL	T1-3a breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized surgical adjuvant trial in 242 evaluable patients with T1-3a , N0-1 , and M0 breast cancer was initiated 4 years ago .
	manualset3
153009	4	408217	13	NULL	NULL	0	NULL	N0-1 breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized surgical adjuvant trial in 242 evaluable patients with T1-3a , N0-1 , and M0 breast cancer was initiated 4 years ago .
	manualset3
153010	5	408217	13	NULL	NULL	0	NULL	M0 breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized surgical adjuvant trial in 242 evaluable patients with T1-3a , N0-1 , and M0 breast cancer was initiated 4 years ago .
	manualset3
153011	6	408217	13	NULL	NULL	0	NULL	4 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized surgical adjuvant trial in 242 evaluable patients with T1-3a , N0-1 , and M0 breast cancer was initiated 4 years ago .
	manualset3
153012	1	408218	13	NULL	NULL	0	NULL	ECG	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The ECG demonstrated deep `` Q '' waves from the inferior leads and inverted `` T '' waves in V1 to V6 , but failed to register arrhythmias .
	manualset3
153013	2	408218	13	NULL	NULL	0	NULL	deep `` Q '' waves	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ECG demonstrated deep `` Q '' waves from the inferior leads and inverted `` T '' waves in V1 to V6 , but failed to register arrhythmias .
	manualset3
153014	3	408218	13	NULL	NULL	0	NULL	leads	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ECG demonstrated deep `` Q '' waves from the inferior leads and inverted `` T '' waves in V1 to V6 , but failed to register arrhythmias .
	manualset3
153015	4	408218	13	NULL	NULL	0	NULL	inverted `` T '' waves	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ECG demonstrated deep `` Q '' waves from the inferior leads and inverted `` T '' waves in V1 to V6 , but failed to register arrhythmias .
	manualset3
153016	5	408218	13	NULL	NULL	0	NULL	V1 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ECG demonstrated deep `` Q '' waves from the inferior leads and inverted `` T '' waves in V1 to V6 , but failed to register arrhythmias .
	manualset3
153017	6	408218	13	NULL	NULL	0	NULL	V6	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ECG demonstrated deep `` Q '' waves from the inferior leads and inverted `` T '' waves in V1 to V6 , but failed to register arrhythmias .
	manualset3
153018	7	408218	13	NULL	NULL	0	NULL	arrhythmias	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The ECG demonstrated deep `` Q '' waves from the inferior leads and inverted `` T '' waves in V1 to V6 , but failed to register arrhythmias .
	manualset3
153021	1	408219	13	NULL	NULL	0	NULL	EEG	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The EEG showed spike and wave discharges over a diffuse slow-wave background activity .
	manualset3
153023	2	408219	13	NULL	NULL	0	NULL	spike discharges	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The EEG showed spike and wave discharges over a diffuse slow-wave background activity .
	manualset3
153024	3	408219	13	NULL	NULL	0	NULL	wave discharges	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The EEG showed spike and wave discharges over a diffuse slow-wave background activity .
	manualset3
153027	4	408219	13	NULL	NULL	0	NULL	slow-wave background activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The EEG showed spike and wave discharges over a diffuse slow-wave background activity .
	manualset3
153035	1	408220	13	NULL	NULL	0	NULL	EGF effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The EGF effect was attenuated by the co-presence of a MEK inhibitor .
	manualset3
153036	2	408220	13	NULL	NULL	0	NULL	co-presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The EGF effect was attenuated by the co-presence of a MEK inhibitor .
	manualset3
153037	3	408220	13	NULL	NULL	0	NULL	MEK inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The EGF effect was attenuated by the co-presence of a MEK inhibitor .
	manualset3
153039	1	408221	13	NULL	NULL	0	NULL	EGFR tyrosine kinase inhibitor 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The EGFR tyrosine kinase inhibitor ( EGFR-TKI ) ZD1839 ( ` Iressa ' ) has clinical activity in a wide range of tumor types , although the mechanism ( s ) by which it exerts its antitumor activity effects remain unclear .
	manualset3
153040	2	408221	13	NULL	NULL	0	NULL	( EGFR-TKI ) ZD1839 ( ` Iressa ' ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The EGFR tyrosine kinase inhibitor ( EGFR-TKI ) ZD1839 ( ` Iressa ' ) has clinical activity in a wide range of tumor types , although the mechanism ( s ) by which it exerts its antitumor activity effects remain unclear .
	manualset3
153041	3	408221	13	NULL	NULL	0	NULL	clinical activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The EGFR tyrosine kinase inhibitor ( EGFR-TKI ) ZD1839 ( ` Iressa ' ) has clinical activity in a wide range of tumor types , although the mechanism ( s ) by which it exerts its antitumor activity effects remain unclear .
	manualset3
153042	4	408221	13	NULL	NULL	0	NULL	wide range of tumor types	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The EGFR tyrosine kinase inhibitor ( EGFR-TKI ) ZD1839 ( ` Iressa ' ) has clinical activity in a wide range of tumor types , although the mechanism ( s ) by which it exerts its antitumor activity effects remain unclear .
	manualset3
153043	5	408221	13	NULL	NULL	0	NULL	mechanism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The EGFR tyrosine kinase inhibitor ( EGFR-TKI ) ZD1839 ( ` Iressa ' ) has clinical activity in a wide range of tumor types , although the mechanism ( s ) by which it exerts its antitumor activity effects remain unclear .
	manualset3
153044	6	408221	13	NULL	NULL	0	NULL	antitumor activity effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The EGFR tyrosine kinase inhibitor ( EGFR-TKI ) ZD1839 ( ` Iressa ' ) has clinical activity in a wide range of tumor types , although the mechanism ( s ) by which it exerts its antitumor activity effects remain unclear .
	manualset3
153055	1	408222	13	NULL	NULL	NULL	NULL	EGIDE unit 	Thing												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The EGIDE unit is considered by its producer to be an alternative for CO2 lasers .
	manualset3
153056	2	408222	13	NULL	NULL	NULL	NULL	producer	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The EGIDE unit is considered by its producer to be an alternative for CO2 lasers .
	manualset3
153057	3	408222	13	NULL	NULL	0	NULL	alternative 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The EGIDE unit is considered by its producer to be an alternative for CO2 lasers .
	manualset3
153059	4	408222	13	NULL	NULL	0	NULL	CO2 lasers	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The EGIDE unit is considered by its producer to be an alternative for CO2 lasers .
	manualset3
153066	1	408223	13	NULL	NULL	0	NULL	 EH	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The EH of FUra in rats at infusion rates ranging from 0.375 to 3 mg/kg/min decreased from 0.750 to 0.225 .
	manualset3
153067	2	408223	13	NULL	NULL	0	NULL	 FUra	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The EH of FUra in rats at infusion rates ranging from 0.375 to 3 mg/kg/min decreased from 0.750 to 0.225 .
	manualset3
153068	3	408223	13	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The EH of FUra in rats at infusion rates ranging from 0.375 to 3 mg/kg/min decreased from 0.750 to 0.225 .
	manualset3
153069	4	408223	13	NULL	NULL	0	NULL	infusion rates 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The EH of FUra in rats at infusion rates ranging from 0.375 to 3 mg/kg/min decreased from 0.750 to 0.225 .
	manualset3
153070	5	408223	13	NULL	NULL	0	NULL	0.375 to 3 mg/kg/min	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The EH of FUra in rats at infusion rates ranging from 0.375 to 3 mg/kg/min decreased from 0.750 to 0.225 .
	manualset3
153072	6	408223	13	NULL	NULL	0	NULL	 0.750 to 0.225	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The EH of FUra in rats at infusion rates ranging from 0.375 to 3 mg/kg/min decreased from 0.750 to 0.225 .
	manualset3
153074	1	408224	13	NULL	NULL	0	NULL	EIA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The EIA for ZEA was in addition used to analyze biological fluids , obtained during a feeding trial .
	manualset3
153075	2	408224	13	NULL	NULL	0	NULL	ZEA  	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The EIA for ZEA was in addition used to analyze biological fluids , obtained during a feeding trial .
	manualset3
153076	3	408224	13	NULL	NULL	0	NULL	biological fluids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The EIA for ZEA was in addition used to analyze biological fluids , obtained during a feeding trial .
	manualset3
153077	4	408224	13	NULL	NULL	0	NULL	feeding trial 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The EIA for ZEA was in addition used to analyze biological fluids , obtained during a feeding trial .
	manualset3
153078	5	408224	13	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The EIA for ZEA was in addition used to analyze biological fluids , obtained during a feeding trial .
	manualset3
153079	1	408225	13	NULL	NULL	0	NULL	 EII 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The EII appears to be most valid in capturing psychiatric severity as measured by researcher ratings of social competency or estimated ego impairment .
	manualset3
153080	2	408225	13	NULL	NULL	0	NULL	psychiatric severity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The EII appears to be most valid in capturing psychiatric severity as measured by researcher ratings of social competency or estimated ego impairment .
	manualset3
153081	3	408225	13	NULL	NULL	0	NULL	researcher ratings 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The EII appears to be most valid in capturing psychiatric severity as measured by researcher ratings of social competency or estimated ego impairment .
	manualset3
153082	4	408225	13	NULL	NULL	0	NULL	social competency 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The EII appears to be most valid in capturing psychiatric severity as measured by researcher ratings of social competency or estimated ego impairment .
	manualset3
153083	5	408225	13	NULL	NULL	0	NULL	ego impairment	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The EII appears to be most valid in capturing psychiatric severity as measured by researcher ratings of social competency or estimated ego impairment .
	manualset3
153089	1	408226	13	NULL	NULL	0	NULL	ELISA test 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ELISA test with anti-turkey conjugate was more sensitive than that with anti-chicken conjugate .
	manualset3
153090	2	408226	13	NULL	NULL	0	NULL	anti-turkey conjugate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ELISA test with anti-turkey conjugate was more sensitive than that with anti-chicken conjugate .
	manualset3
153091	3	408226	13	NULL	NULL	0	NULL	anti-chicken conjugate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ELISA test with anti-turkey conjugate was more sensitive than that with anti-chicken conjugate .
	manualset3
153097	1	408227	13	NULL	NULL	NULL	NULL	EST	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The EST on developmental neurontoxicity could be applied to the safety evaluation in vitro .
	manualset3
153098	2	408227	13	NULL	NULL	0	NULL	developmental neurontoxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The EST on developmental neurontoxicity could be applied to the safety evaluation in vitro .
	manualset3
153100	3	408227	13	NULL	NULL	NULL	NULL	safety evaluation 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The EST on developmental neurontoxicity could be applied to the safety evaluation in vitro .
	manualset3
153103	1	408228	13	NULL	NULL	0	NULL	ESTRIPc program	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The ESTRIPc program , developed for pharmacokinetic analysis and modified for the study of bacterial clearance , was employed to fit the experimental data of bacterial survival versus time to a polyexponential equation with 1 , 2 , or 3 terms .
	manualset3
153105	2	408228	13	NULL	NULL	0	NULL	pharmacokinetic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ESTRIPc program , developed for pharmacokinetic analysis and modified for the study of bacterial clearance , was employed to fit the experimental data of bacterial survival versus time to a polyexponential equation with 1 , 2 , or 3 terms .
	manualset3
153106	3	408228	13	NULL	NULL	NULL	NULL	study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ESTRIPc program , developed for pharmacokinetic analysis and modified for the study of bacterial clearance , was employed to fit the experimental data of bacterial survival versus time to a polyexponential equation with 1 , 2 , or 3 terms .
	manualset3
153107	4	408228	13	NULL	NULL	0	NULL	bacterial clearance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ESTRIPc program , developed for pharmacokinetic analysis and modified for the study of bacterial clearance , was employed to fit the experimental data of bacterial survival versus time to a polyexponential equation with 1 , 2 , or 3 terms .
	manualset3
153109	5	408228	13	NULL	NULL	0	NULL	experimental data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The ESTRIPc program , developed for pharmacokinetic analysis and modified for the study of bacterial clearance , was employed to fit the experimental data of bacterial survival versus time to a polyexponential equation with 1 , 2 , or 3 terms .
	manualset3
153110	6	408228	13	NULL	NULL	0	NULL	 bacterial survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ESTRIPc program , developed for pharmacokinetic analysis and modified for the study of bacterial clearance , was employed to fit the experimental data of bacterial survival versus time to a polyexponential equation with 1 , 2 , or 3 terms .
	manualset3
153112	7	408228	13	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The ESTRIPc program , developed for pharmacokinetic analysis and modified for the study of bacterial clearance , was employed to fit the experimental data of bacterial survival versus time to a polyexponential equation with 1 , 2 , or 3 terms .
	manualset3
153113	8	408228	13	NULL	NULL	0	NULL	polyexponential equation	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The ESTRIPc program , developed for pharmacokinetic analysis and modified for the study of bacterial clearance , was employed to fit the experimental data of bacterial survival versus time to a polyexponential equation with 1 , 2 , or 3 terms .
	manualset3
153115	9	408228	13	NULL	NULL	NULL	NULL	1 term	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ESTRIPc program , developed for pharmacokinetic analysis and modified for the study of bacterial clearance , was employed to fit the experimental data of bacterial survival versus time to a polyexponential equation with 1 , 2 , or 3 terms .
	manualset3
153117	10	408228	13	NULL	NULL	0	NULL	2 terms	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ESTRIPc program , developed for pharmacokinetic analysis and modified for the study of bacterial clearance , was employed to fit the experimental data of bacterial survival versus time to a polyexponential equation with 1 , 2 , or 3 terms .
	manualset3
153118	11	408228	13	NULL	NULL	0	NULL	3 terms 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ESTRIPc program , developed for pharmacokinetic analysis and modified for the study of bacterial clearance , was employed to fit the experimental data of bacterial survival versus time to a polyexponential equation with 1 , 2 , or 3 terms .
	manualset3
153122	1	408229	13	NULL	NULL	0	NULL	ET task	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ET task required subjects to initiate movements in response to consecutive visual cues ; the SI task allowed them to start at will .
	manualset3
153124	2	408229	13	NULL	NULL	0	NULL	subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The ET task required subjects to initiate movements in response to consecutive visual cues ; the SI task allowed them to start at will .
	manualset3
153126	3	408229	13	NULL	NULL	0	NULL	movements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ET task required subjects to initiate movements in response to consecutive visual cues ; the SI task allowed them to start at will .
	manualset3
153127	4	408229	13	NULL	NULL	0	NULL	response	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ET task required subjects to initiate movements in response to consecutive visual cues ; the SI task allowed them to start at will .
	manualset3
153128	5	408229	13	NULL	NULL	0	NULL	consecutive visual cues 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ET task required subjects to initiate movements in response to consecutive visual cues ; the SI task allowed them to start at will .
	manualset3
153135	6	408229	13	NULL	NULL	0	NULL	SI task	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ET task required subjects to initiate movements in response to consecutive visual cues ; the SI task allowed them to start at will .
	manualset3
153136	1	408230	13	NULL	NULL	0	NULL	Effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Effect of Hydrogen-Ion Concentration on Locomotion and Other Life-Processes in Amoeba Proteus .
	manualset3
153137	2	408230	13	NULL	NULL	0	NULL	Hydrogen-Ion Concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Effect of Hydrogen-Ion Concentration on Locomotion and Other Life-Processes in Amoeba Proteus .
	manualset3
153138	3	408230	13	NULL	NULL	0	NULL	 Locomotion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Effect of Hydrogen-Ion Concentration on Locomotion and Other Life-Processes in Amoeba Proteus .
	manualset3
153139	4	408230	13	NULL	NULL	0	NULL	Life-Processes 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Effect of Hydrogen-Ion Concentration on Locomotion and Other Life-Processes in Amoeba Proteus .
	manualset3
153140	5	408230	13	NULL	NULL	0	NULL	Amoeba Proteus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The Effect of Hydrogen-Ion Concentration on Locomotion and Other Life-Processes in Amoeba Proteus .
	manualset3
153141	1	408231	13	NULL	NULL	0	NULL	 Effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Effects of the Inhalation of Coal and Stone Dusts on the Lungs of Pit Ponies .
	manualset3
153142	2	408231	13	NULL	NULL	0	NULL	 Inhalation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Effects of the Inhalation of Coal and Stone Dusts on the Lungs of Pit Ponies .
	manualset3
153143	3	408231	13	NULL	NULL	0	NULL	Coal	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The Effects of the Inhalation of Coal and Stone Dusts on the Lungs of Pit Ponies .
	manualset3
153144	4	408231	13	NULL	NULL	0	NULL	Stone Dusts 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The Effects of the Inhalation of Coal and Stone Dusts on the Lungs of Pit Ponies .
	manualset3
153145	5	408231	13	NULL	NULL	0	NULL	Lungs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The Effects of the Inhalation of Coal and Stone Dusts on the Lungs of Pit Ponies .
	manualset3
153146	6	408231	13	NULL	NULL	0	NULL	Pit Ponies	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The Effects of the Inhalation of Coal and Stone Dusts on the Lungs of Pit Ponies .
	manualset3
153147	1	408232	13	NULL	NULL	0	NULL	Ensemble/Legacy Chimera extension	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The Ensemble/Legacy Chimera extension : standardized user and programmer interface to molecular Ensemble data and Legacy modeling programs .
	manualset3
153148	2	408232	13	NULL	NULL	0	NULL	user 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The Ensemble/Legacy Chimera extension : standardized user and programmer interface to molecular Ensemble data and Legacy modeling programs .
	manualset3
153149	3	408232	13	NULL	NULL	NULL	NULL	programmer interface	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The Ensemble/Legacy Chimera extension : standardized user and programmer interface to molecular Ensemble data and Legacy modeling programs .
	manualset3
153150	4	408232	13	NULL	NULL	0	NULL	molecular Ensemble data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The Ensemble/Legacy Chimera extension : standardized user and programmer interface to molecular Ensemble data and Legacy modeling programs .
	manualset3
153151	5	408232	13	NULL	NULL	0	NULL	Legacy modeling programs	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The Ensemble/Legacy Chimera extension : standardized user and programmer interface to molecular Ensemble data and Legacy modeling programs .
	manualset3
153152	1	408233	13	NULL	NULL	0	NULL	Entomophthorales 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The Entomophthorales are closely related to the Mucorales on the basis of sexual growth by production of zygospores and by the production of coenocytic hyphae .
	manualset3
153153	2	408233	13	NULL	NULL	0	NULL	Mucorales	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The Entomophthorales are closely related to the Mucorales on the basis of sexual growth by production of zygospores and by the production of coenocytic hyphae .
	manualset3
153154	3	408233	13	NULL	NULL	0	NULL	basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Entomophthorales are closely related to the Mucorales on the basis of sexual growth by production of zygospores and by the production of coenocytic hyphae .
	manualset3
153155	4	408233	13	NULL	NULL	0	NULL	sexual growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Entomophthorales are closely related to the Mucorales on the basis of sexual growth by production of zygospores and by the production of coenocytic hyphae .
	manualset3
153156	5	408233	13	NULL	NULL	0	NULL	production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Entomophthorales are closely related to the Mucorales on the basis of sexual growth by production of zygospores and by the production of coenocytic hyphae .
	manualset3
153157	6	408233	13	NULL	NULL	0	NULL	zygospores	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The Entomophthorales are closely related to the Mucorales on the basis of sexual growth by production of zygospores and by the production of coenocytic hyphae .
	manualset3
153158	7	408233	13	NULL	NULL	0	NULL	production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Entomophthorales are closely related to the Mucorales on the basis of sexual growth by production of zygospores and by the production of coenocytic hyphae .
	manualset3
153159	8	408233	13	NULL	NULL	0	NULL	 coenocytic hyphae	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The Entomophthorales are closely related to the Mucorales on the basis of sexual growth by production of zygospores and by the production of coenocytic hyphae .
	manualset3
153160	1	408234	13	NULL	NULL	0	NULL	Eu3 + release assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Eu3 + release assay was then used to measure NK and LAK activities in the peripheral blood of women with cervical SIL or cervical squamous cell carcinoma ( SCC ) .
	manualset3
153161	2	408234	13	NULL	NULL	0	NULL	NK activities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Eu3 + release assay was then used to measure NK and LAK activities in the peripheral blood of women with cervical SIL or cervical squamous cell carcinoma ( SCC ) .
	manualset3
153162	3	408234	13	NULL	NULL	0	NULL	LAK activities 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Eu3 + release assay was then used to measure NK and LAK activities in the peripheral blood of women with cervical SIL or cervical squamous cell carcinoma ( SCC ) .
	manualset3
153163	4	408234	13	NULL	NULL	0	NULL	peripheral blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The Eu3 + release assay was then used to measure NK and LAK activities in the peripheral blood of women with cervical SIL or cervical squamous cell carcinoma ( SCC ) .
	manualset3
153164	5	408234	13	NULL	NULL	0	NULL	 women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The Eu3 + release assay was then used to measure NK and LAK activities in the peripheral blood of women with cervical SIL or cervical squamous cell carcinoma ( SCC ) .
	manualset3
153165	6	408234	13	NULL	NULL	0	NULL	cervical SIL	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The Eu3 + release assay was then used to measure NK and LAK activities in the peripheral blood of women with cervical SIL or cervical squamous cell carcinoma ( SCC ) .
	manualset3
153166	7	408234	13	NULL	NULL	0	NULL	cervical squamous cell carcinoma ( SCC ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The Eu3 + release assay was then used to measure NK and LAK activities in the peripheral blood of women with cervical SIL or cervical squamous cell carcinoma ( SCC ) .
	manualset3
153167	1	408235	13	NULL	NULL	0	NULL	trial	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized trial of combined modality therapy employing combination chemotherapy ( cyclophosphamide ( CTX ) and methotrexate ( MTX ) , CTX , MTX and Vincristine ( VCR ) and CTX , VCR and high-dose MTX with citrovorum rescue ) and radiation therapy was compared to cyclophosphamide and radiation therapy in 258 patients with pulmonary small cell carcinoma .
	manualset3
153168	2	408235	13	NULL	NULL	0	NULL	modality therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized trial of combined modality therapy employing combination chemotherapy ( cyclophosphamide ( CTX ) and methotrexate ( MTX ) , CTX , MTX and Vincristine ( VCR ) and CTX , VCR and high-dose MTX with citrovorum rescue ) and radiation therapy was compared to cyclophosphamide and radiation therapy in 258 patients with pulmonary small cell carcinoma .
	manualset3
153169	3	408235	13	NULL	NULL	0	NULL	combination chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized trial of combined modality therapy employing combination chemotherapy ( cyclophosphamide ( CTX ) and methotrexate ( MTX ) , CTX , MTX and Vincristine ( VCR ) and CTX , VCR and high-dose MTX with citrovorum rescue ) and radiation therapy was compared to cyclophosphamide and radiation therapy in 258 patients with pulmonary small cell carcinoma .
	manualset3
153170	4	408235	13	NULL	NULL	0	NULL	cyclophosphamide ( CTX )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized trial of combined modality therapy employing combination chemotherapy ( cyclophosphamide ( CTX ) and methotrexate ( MTX ) , CTX , MTX and Vincristine ( VCR ) and CTX , VCR and high-dose MTX with citrovorum rescue ) and radiation therapy was compared to cyclophosphamide and radiation therapy in 258 patients with pulmonary small cell carcinoma .
	manualset3
153171	5	408235	13	NULL	NULL	0	NULL	methotrexate ( MTX )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized trial of combined modality therapy employing combination chemotherapy ( cyclophosphamide ( CTX ) and methotrexate ( MTX ) , CTX , MTX and Vincristine ( VCR ) and CTX , VCR and high-dose MTX with citrovorum rescue ) and radiation therapy was compared to cyclophosphamide and radiation therapy in 258 patients with pulmonary small cell carcinoma .
	manualset3
153172	6	408235	13	NULL	NULL	0	NULL	CTX	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized trial of combined modality therapy employing combination chemotherapy ( cyclophosphamide ( CTX ) and methotrexate ( MTX ) , CTX , MTX and Vincristine ( VCR ) and CTX , VCR and high-dose MTX with citrovorum rescue ) and radiation therapy was compared to cyclophosphamide and radiation therapy in 258 patients with pulmonary small cell carcinoma .
	manualset3
153173	7	408235	13	NULL	NULL	0	NULL	MTX	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized trial of combined modality therapy employing combination chemotherapy ( cyclophosphamide ( CTX ) and methotrexate ( MTX ) , CTX , MTX and Vincristine ( VCR ) and CTX , VCR and high-dose MTX with citrovorum rescue ) and radiation therapy was compared to cyclophosphamide and radiation therapy in 258 patients with pulmonary small cell carcinoma .
	manualset3
153174	8	408235	13	NULL	NULL	0	NULL	Vincristine ( VCR )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized trial of combined modality therapy employing combination chemotherapy ( cyclophosphamide ( CTX ) and methotrexate ( MTX ) , CTX , MTX and Vincristine ( VCR ) and CTX , VCR and high-dose MTX with citrovorum rescue ) and radiation therapy was compared to cyclophosphamide and radiation therapy in 258 patients with pulmonary small cell carcinoma .
	manualset3
153175	9	408235	13	NULL	NULL	0	NULL	CTX	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized trial of combined modality therapy employing combination chemotherapy ( cyclophosphamide ( CTX ) and methotrexate ( MTX ) , CTX , MTX and Vincristine ( VCR ) and CTX , VCR and high-dose MTX with citrovorum rescue ) and radiation therapy was compared to cyclophosphamide and radiation therapy in 258 patients with pulmonary small cell carcinoma .
	manualset3
153176	10	408235	13	NULL	NULL	0	NULL	VCR	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized trial of combined modality therapy employing combination chemotherapy ( cyclophosphamide ( CTX ) and methotrexate ( MTX ) , CTX , MTX and Vincristine ( VCR ) and CTX , VCR and high-dose MTX with citrovorum rescue ) and radiation therapy was compared to cyclophosphamide and radiation therapy in 258 patients with pulmonary small cell carcinoma .
	manualset3
153177	11	408235	13	NULL	NULL	0	NULL	MTX 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized trial of combined modality therapy employing combination chemotherapy ( cyclophosphamide ( CTX ) and methotrexate ( MTX ) , CTX , MTX and Vincristine ( VCR ) and CTX , VCR and high-dose MTX with citrovorum rescue ) and radiation therapy was compared to cyclophosphamide and radiation therapy in 258 patients with pulmonary small cell carcinoma .
	manualset3
153178	12	408235	13	NULL	NULL	0	NULL	citrovorum rescue	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized trial of combined modality therapy employing combination chemotherapy ( cyclophosphamide ( CTX ) and methotrexate ( MTX ) , CTX , MTX and Vincristine ( VCR ) and CTX , VCR and high-dose MTX with citrovorum rescue ) and radiation therapy was compared to cyclophosphamide and radiation therapy in 258 patients with pulmonary small cell carcinoma .
	manualset3
153179	13	408235	13	NULL	NULL	0	NULL	radiation therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized trial of combined modality therapy employing combination chemotherapy ( cyclophosphamide ( CTX ) and methotrexate ( MTX ) , CTX , MTX and Vincristine ( VCR ) and CTX , VCR and high-dose MTX with citrovorum rescue ) and radiation therapy was compared to cyclophosphamide and radiation therapy in 258 patients with pulmonary small cell carcinoma .
	manualset3
153180	14	408235	13	NULL	NULL	0	NULL	cyclophosphamide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized trial of combined modality therapy employing combination chemotherapy ( cyclophosphamide ( CTX ) and methotrexate ( MTX ) , CTX , MTX and Vincristine ( VCR ) and CTX , VCR and high-dose MTX with citrovorum rescue ) and radiation therapy was compared to cyclophosphamide and radiation therapy in 258 patients with pulmonary small cell carcinoma .
	manualset3
153181	15	408235	13	NULL	NULL	0	NULL	radiation therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized trial of combined modality therapy employing combination chemotherapy ( cyclophosphamide ( CTX ) and methotrexate ( MTX ) , CTX , MTX and Vincristine ( VCR ) and CTX , VCR and high-dose MTX with citrovorum rescue ) and radiation therapy was compared to cyclophosphamide and radiation therapy in 258 patients with pulmonary small cell carcinoma .
	manualset3
153182	16	408235	13	NULL	NULL	0	NULL	258 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized trial of combined modality therapy employing combination chemotherapy ( cyclophosphamide ( CTX ) and methotrexate ( MTX ) , CTX , MTX and Vincristine ( VCR ) and CTX , VCR and high-dose MTX with citrovorum rescue ) and radiation therapy was compared to cyclophosphamide and radiation therapy in 258 patients with pulmonary small cell carcinoma .
	manualset3
153183	17	408235	13	NULL	NULL	0	NULL	pulmonary small cell carcinoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A randomized trial of combined modality therapy employing combination chemotherapy ( cyclophosphamide ( CTX ) and methotrexate ( MTX ) , CTX , MTX and Vincristine ( VCR ) and CTX , VCR and high-dose MTX with citrovorum rescue ) and radiation therapy was compared to cyclophosphamide and radiation therapy in 258 patients with pulmonary small cell carcinoma .
	manualset3
153184	1	408236	13	NULL	NULL	0	NULL	F. oxysporum PHR1 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The F. oxysporum PHR1 protein has a domain characteristic of photolyases from fungi ( Trichoderma harziaium , N. crassa , Magnaporthe grisea , Saccharomyces cerevisiae ) to bacteria ( E. coli ) , and clusters in the photolyases phylogenetic tree with fungal photolyases .
	manualset3
153185	2	408236	13	NULL	NULL	0	NULL	domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The F. oxysporum PHR1 protein has a domain characteristic of photolyases from fungi ( Trichoderma harziaium , N. crassa , Magnaporthe grisea , Saccharomyces cerevisiae ) to bacteria ( E. coli ) , and clusters in the photolyases phylogenetic tree with fungal photolyases .
	manualset3
153186	3	408236	13	NULL	NULL	0	NULL	photolyases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The F. oxysporum PHR1 protein has a domain characteristic of photolyases from fungi ( Trichoderma harziaium , N. crassa , Magnaporthe grisea , Saccharomyces cerevisiae ) to bacteria ( E. coli ) , and clusters in the photolyases phylogenetic tree with fungal photolyases .
	manualset3
153187	4	408236	13	NULL	NULL	0	NULL	fungi	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The F. oxysporum PHR1 protein has a domain characteristic of photolyases from fungi ( Trichoderma harziaium , N. crassa , Magnaporthe grisea , Saccharomyces cerevisiae ) to bacteria ( E. coli ) , and clusters in the photolyases phylogenetic tree with fungal photolyases .
	manualset3
153188	5	408236	13	NULL	NULL	0	NULL	Trichoderma harziaium	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The F. oxysporum PHR1 protein has a domain characteristic of photolyases from fungi ( Trichoderma harziaium , N. crassa , Magnaporthe grisea , Saccharomyces cerevisiae ) to bacteria ( E. coli ) , and clusters in the photolyases phylogenetic tree with fungal photolyases .
	manualset3
153189	6	408236	13	NULL	NULL	0	NULL	N. crassa	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The F. oxysporum PHR1 protein has a domain characteristic of photolyases from fungi ( Trichoderma harziaium , N. crassa , Magnaporthe grisea , Saccharomyces cerevisiae ) to bacteria ( E. coli ) , and clusters in the photolyases phylogenetic tree with fungal photolyases .
	manualset3
153190	7	408236	13	NULL	NULL	0	NULL	Magnaporthe grisea	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The F. oxysporum PHR1 protein has a domain characteristic of photolyases from fungi ( Trichoderma harziaium , N. crassa , Magnaporthe grisea , Saccharomyces cerevisiae ) to bacteria ( E. coli ) , and clusters in the photolyases phylogenetic tree with fungal photolyases .
	manualset3
153191	8	408236	13	NULL	NULL	0	NULL	Saccharomyces cerevisiae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The F. oxysporum PHR1 protein has a domain characteristic of photolyases from fungi ( Trichoderma harziaium , N. crassa , Magnaporthe grisea , Saccharomyces cerevisiae ) to bacteria ( E. coli ) , and clusters in the photolyases phylogenetic tree with fungal photolyases .
	manualset3
153192	9	408236	13	NULL	NULL	0	NULL	 bacteria 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The F. oxysporum PHR1 protein has a domain characteristic of photolyases from fungi ( Trichoderma harziaium , N. crassa , Magnaporthe grisea , Saccharomyces cerevisiae ) to bacteria ( E. coli ) , and clusters in the photolyases phylogenetic tree with fungal photolyases .
	manualset3
153193	10	408236	13	NULL	NULL	0	NULL	E. coli 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The F. oxysporum PHR1 protein has a domain characteristic of photolyases from fungi ( Trichoderma harziaium , N. crassa , Magnaporthe grisea , Saccharomyces cerevisiae ) to bacteria ( E. coli ) , and clusters in the photolyases phylogenetic tree with fungal photolyases .
	manualset3
153194	11	408236	13	NULL	NULL	0	NULL	clusters	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The F. oxysporum PHR1 protein has a domain characteristic of photolyases from fungi ( Trichoderma harziaium , N. crassa , Magnaporthe grisea , Saccharomyces cerevisiae ) to bacteria ( E. coli ) , and clusters in the photolyases phylogenetic tree with fungal photolyases .
	manualset3
153195	12	408236	13	NULL	NULL	0	NULL	photolyases phylogenetic tree	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The F. oxysporum PHR1 protein has a domain characteristic of photolyases from fungi ( Trichoderma harziaium , N. crassa , Magnaporthe grisea , Saccharomyces cerevisiae ) to bacteria ( E. coli ) , and clusters in the photolyases phylogenetic tree with fungal photolyases .
	manualset3
153196	13	408236	13	NULL	NULL	0	NULL	fungal photolyases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The F. oxysporum PHR1 protein has a domain characteristic of photolyases from fungi ( Trichoderma harziaium , N. crassa , Magnaporthe grisea , Saccharomyces cerevisiae ) to bacteria ( E. coli ) , and clusters in the photolyases phylogenetic tree with fungal photolyases .
	manualset3
153197	1	408237	13	NULL	NULL	0	NULL	F13L ( p37 ) - deleted ( and ST-246 resistant ) vaccinia virus recombinant ( Vac-F13L ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The F13L ( p37 ) - deleted ( and ST-246 resistant ) vaccinia virus recombinant ( Vac-F13L ) produced smaller plaques than the wild-type vaccinia ( Western Reserve vaccinia ) .
	manualset3
153198	2	408237	13	NULL	NULL	0	NULL	smaller plaques	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The F13L ( p37 ) - deleted ( and ST-246 resistant ) vaccinia virus recombinant ( Vac-F13L ) produced smaller plaques than the wild-type vaccinia ( Western Reserve vaccinia ) .
	manualset3
153199	3	408237	13	NULL	NULL	0	NULL	wild-type vaccinia	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The F13L ( p37 ) - deleted ( and ST-246 resistant ) vaccinia virus recombinant ( Vac-F13L ) produced smaller plaques than the wild-type vaccinia ( Western Reserve vaccinia ) .
	manualset3
153200	4	408237	13	NULL	NULL	0	NULL	Western Reserve vaccinia 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The F13L ( p37 ) - deleted ( and ST-246 resistant ) vaccinia virus recombinant ( Vac-F13L ) produced smaller plaques than the wild-type vaccinia ( Western Reserve vaccinia ) .
	manualset3
153201	1	408238	13	NULL	NULL	NULL	NULL	 FAEE concentrations	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The FAEE concentrations of negative ( 95 % confidence interval , 0.38-0 .49 nmol/g ) versus positive ( 95 % confidence interval , 7.74-151 .28 nmol/g ) samples were distinct , further demonstrating the specificity of this biomarker in determining significant prenatal ethanol exposure .
	manualset3
153202	2	408238	13	NULL	NULL	0	NULL	95 % confidence interval 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The FAEE concentrations of negative ( 95 % confidence interval , 0.38-0 .49 nmol/g ) versus positive ( 95 % confidence interval , 7.74-151 .28 nmol/g ) samples were distinct , further demonstrating the specificity of this biomarker in determining significant prenatal ethanol exposure .
	manualset3
153203	3	408238	13	NULL	NULL	0	NULL	0.38-0 .49 nmol/g	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The FAEE concentrations of negative ( 95 % confidence interval , 0.38-0 .49 nmol/g ) versus positive ( 95 % confidence interval , 7.74-151 .28 nmol/g ) samples were distinct , further demonstrating the specificity of this biomarker in determining significant prenatal ethanol exposure .
	manualset3
153204	4	408238	13	NULL	NULL	0	NULL	 95 % confidence interval	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The FAEE concentrations of negative ( 95 % confidence interval , 0.38-0 .49 nmol/g ) versus positive ( 95 % confidence interval , 7.74-151 .28 nmol/g ) samples were distinct , further demonstrating the specificity of this biomarker in determining significant prenatal ethanol exposure .
	manualset3
153205	5	408238	13	NULL	NULL	0	NULL	7.74-151 .28 nmol/g 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The FAEE concentrations of negative ( 95 % confidence interval , 0.38-0 .49 nmol/g ) versus positive ( 95 % confidence interval , 7.74-151 .28 nmol/g ) samples were distinct , further demonstrating the specificity of this biomarker in determining significant prenatal ethanol exposure .
	manualset3
153206	6	408238	13	NULL	NULL	0	NULL	samples	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The FAEE concentrations of negative ( 95 % confidence interval , 0.38-0 .49 nmol/g ) versus positive ( 95 % confidence interval , 7.74-151 .28 nmol/g ) samples were distinct , further demonstrating the specificity of this biomarker in determining significant prenatal ethanol exposure .
	manualset3
153207	7	408238	13	NULL	NULL	0	NULL	specificity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The FAEE concentrations of negative ( 95 % confidence interval , 0.38-0 .49 nmol/g ) versus positive ( 95 % confidence interval , 7.74-151 .28 nmol/g ) samples were distinct , further demonstrating the specificity of this biomarker in determining significant prenatal ethanol exposure .
	manualset3
153208	8	408238	13	NULL	NULL	0	NULL	biomarker 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The FAEE concentrations of negative ( 95 % confidence interval , 0.38-0 .49 nmol/g ) versus positive ( 95 % confidence interval , 7.74-151 .28 nmol/g ) samples were distinct , further demonstrating the specificity of this biomarker in determining significant prenatal ethanol exposure .
	manualset3
153209	9	408238	13	NULL	NULL	0	NULL	prenatal ethanol exposure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The FAEE concentrations of negative ( 95 % confidence interval , 0.38-0 .49 nmol/g ) versus positive ( 95 % confidence interval , 7.74-151 .28 nmol/g ) samples were distinct , further demonstrating the specificity of this biomarker in determining significant prenatal ethanol exposure .
	manualset3
153210	1	408239	13	NULL	NULL	0	NULL	FIA-SWAdSV method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The FIA-SWAdSV method enabled analysis of up to 120 samples per hour at reduced cost , implying the possibility of competing with the chromatographic methods usually used for this analysis .
	manualset3
153211	2	408239	13	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The FIA-SWAdSV method enabled analysis of up to 120 samples per hour at reduced cost , implying the possibility of competing with the chromatographic methods usually used for this analysis .
	manualset3
153212	3	408239	13	NULL	NULL	0	NULL	120 samples per hour	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The FIA-SWAdSV method enabled analysis of up to 120 samples per hour at reduced cost , implying the possibility of competing with the chromatographic methods usually used for this analysis .
	manualset3
153213	4	408239	13	NULL	NULL	0	NULL	cost	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The FIA-SWAdSV method enabled analysis of up to 120 samples per hour at reduced cost , implying the possibility of competing with the chromatographic methods usually used for this analysis .
	manualset3
153214	5	408239	13	NULL	NULL	0	NULL	possibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The FIA-SWAdSV method enabled analysis of up to 120 samples per hour at reduced cost , implying the possibility of competing with the chromatographic methods usually used for this analysis .
	manualset3
153215	6	408239	13	NULL	NULL	0	NULL	chromatographic methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The FIA-SWAdSV method enabled analysis of up to 120 samples per hour at reduced cost , implying the possibility of competing with the chromatographic methods usually used for this analysis .
	manualset3
153216	7	408239	13	NULL	NULL	0	NULL	analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The FIA-SWAdSV method enabled analysis of up to 120 samples per hour at reduced cost , implying the possibility of competing with the chromatographic methods usually used for this analysis .
	manualset3
153217	1	408240	13	NULL	NULL	0	NULL	FM+EC grafts	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The FM+EC grafts induced more endothelialization than those seeded with ECs alone .
	manualset3
153218	2	408240	13	NULL	NULL	0	NULL	endothelialization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The FM+EC grafts induced more endothelialization than those seeded with ECs alone .
	manualset3
153219	3	408240	13	NULL	NULL	0	NULL	ECs	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The FM+EC grafts induced more endothelialization than those seeded with ECs alone .
	manualset3
153220	1	408241	13	NULL	NULL	0	NULL	FSR 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The FSR of palmitate from acetate was 5.2 % per day .
	manualset3
153221	2	408241	13	NULL	NULL	0	NULL	palmitate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The FSR of palmitate from acetate was 5.2 % per day .
	manualset3
153222	3	408241	13	NULL	NULL	0	NULL	acetate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The FSR of palmitate from acetate was 5.2 % per day .
	manualset3
153223	4	408241	13	NULL	NULL	0	NULL	5.2 % per day	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The FSR of palmitate from acetate was 5.2 % per day .
	manualset3
153224	1	408242	13	NULL	NULL	0	NULL	FSW	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The FSW are older , less educated , unmarried , staying away from home , speak Kannada with 60 per cent using condoms for preventing pregnancy .
	manualset3
153225	2	408242	13	NULL	NULL	0	NULL	home	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The FSW are older , less educated , unmarried , staying away from home , speak Kannada with 60 per cent using condoms for preventing pregnancy .
	manualset3
153226	3	408242	13	NULL	NULL	0	NULL	Kannada 	Language												NULL		0	NULL	NULL	NULL	NULL	NULL	The FSW are older , less educated , unmarried , staying away from home , speak Kannada with 60 per cent using condoms for preventing pregnancy .
	manualset3
153227	4	408242	13	NULL	NULL	0	NULL	60 per cent	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The FSW are older , less educated , unmarried , staying away from home , speak Kannada with 60 per cent using condoms for preventing pregnancy .
	manualset3
153228	5	408242	13	NULL	NULL	0	NULL	condoms	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The FSW are older , less educated , unmarried , staying away from home , speak Kannada with 60 per cent using condoms for preventing pregnancy .
	manualset3
153229	6	408242	13	NULL	NULL	0	NULL	pregnancy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The FSW are older , less educated , unmarried , staying away from home , speak Kannada with 60 per cent using condoms for preventing pregnancy .
	manualset3
153230	1	408243	13	NULL	NULL	0	NULL	FWMFs	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The FWMFs were not only comparable with those reported for other Arctic marine food webs but also with quite different food webs such as freshwater lakes in the sub-Arctic , East Africa and Papua New Guinea .
	manualset3
153231	2	408243	13	NULL	NULL	0	NULL	Arctic marine food webs	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The FWMFs were not only comparable with those reported for other Arctic marine food webs but also with quite different food webs such as freshwater lakes in the sub-Arctic , East Africa and Papua New Guinea .
	manualset3
153232	3	408243	13	NULL	NULL	0	NULL	 food webs	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The FWMFs were not only comparable with those reported for other Arctic marine food webs but also with quite different food webs such as freshwater lakes in the sub-Arctic , East Africa and Papua New Guinea .
	manualset3
153233	4	408243	13	NULL	NULL	0	NULL	 freshwater lakes	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The FWMFs were not only comparable with those reported for other Arctic marine food webs but also with quite different food webs such as freshwater lakes in the sub-Arctic , East Africa and Papua New Guinea .
	manualset3
153234	5	408243	13	NULL	NULL	0	NULL	sub-Arctic	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The FWMFs were not only comparable with those reported for other Arctic marine food webs but also with quite different food webs such as freshwater lakes in the sub-Arctic , East Africa and Papua New Guinea .
	manualset3
153235	6	408243	13	NULL	NULL	0	NULL	East Africa	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The FWMFs were not only comparable with those reported for other Arctic marine food webs but also with quite different food webs such as freshwater lakes in the sub-Arctic , East Africa and Papua New Guinea .
	manualset3
153236	7	408243	13	NULL	NULL	0	NULL	Papua New Guinea	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The FWMFs were not only comparable with those reported for other Arctic marine food webs but also with quite different food webs such as freshwater lakes in the sub-Arctic , East Africa and Papua New Guinea .
	manualset3
153237	1	408244	13	NULL	NULL	0	NULL	range	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A range of cis complexes of zirconium with the 2 , 2 ' - diaminobibenzyl ( C6-chain ) backbone give low to moderate productivities of multimodal poly ( ethene ) , while in contrast the structurally analogous titanium compounds provide highly active , single site catalysts .
	manualset3
153238	2	408244	13	NULL	NULL	0	NULL	cis complexes of zirconium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A range of cis complexes of zirconium with the 2 , 2 ' - diaminobibenzyl ( C6-chain ) backbone give low to moderate productivities of multimodal poly ( ethene ) , while in contrast the structurally analogous titanium compounds provide highly active , single site catalysts .
	manualset3
153239	3	408244	13	NULL	NULL	0	NULL	2 , 2 ' - diaminobibenzyl ( C6-chain ) backbone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A range of cis complexes of zirconium with the 2 , 2 ' - diaminobibenzyl ( C6-chain ) backbone give low to moderate productivities of multimodal poly ( ethene ) , while in contrast the structurally analogous titanium compounds provide highly active , single site catalysts .
	manualset3
153240	4	408244	13	NULL	NULL	NULL	NULL	productivities 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A range of cis complexes of zirconium with the 2 , 2 ' - diaminobibenzyl ( C6-chain ) backbone give low to moderate productivities of multimodal poly ( ethene ) , while in contrast the structurally analogous titanium compounds provide highly active , single site catalysts .
	manualset3
153241	5	408244	13	NULL	NULL	0	NULL	multimodal poly ( ethene ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A range of cis complexes of zirconium with the 2 , 2 ' - diaminobibenzyl ( C6-chain ) backbone give low to moderate productivities of multimodal poly ( ethene ) , while in contrast the structurally analogous titanium compounds provide highly active , single site catalysts .
	manualset3
153242	6	408244	13	NULL	NULL	0	NULL	contrast	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A range of cis complexes of zirconium with the 2 , 2 ' - diaminobibenzyl ( C6-chain ) backbone give low to moderate productivities of multimodal poly ( ethene ) , while in contrast the structurally analogous titanium compounds provide highly active , single site catalysts .
	manualset3
153243	7	408244	13	NULL	NULL	0	NULL	titanium compounds 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A range of cis complexes of zirconium with the 2 , 2 ' - diaminobibenzyl ( C6-chain ) backbone give low to moderate productivities of multimodal poly ( ethene ) , while in contrast the structurally analogous titanium compounds provide highly active , single site catalysts .
	manualset3
153244	8	408244	13	NULL	NULL	0	NULL	single site catalysts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A range of cis complexes of zirconium with the 2 , 2 ' - diaminobibenzyl ( C6-chain ) backbone give low to moderate productivities of multimodal poly ( ethene ) , while in contrast the structurally analogous titanium compounds provide highly active , single site catalysts .
	manualset3
153245	1	408245	13	NULL	NULL	0	NULL	FeLV-infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The FeLV-infection may lead to fatal diseases in domestic and small wild cats .
	manualset3
153246	2	408245	13	NULL	NULL	0	NULL	fatal diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The FeLV-infection may lead to fatal diseases in domestic and small wild cats .
	manualset3
153247	3	408245	13	NULL	NULL	0	NULL	domestic cats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The FeLV-infection may lead to fatal diseases in domestic and small wild cats .
	manualset3
153248	4	408245	13	NULL	NULL	0	NULL	small wild cats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The FeLV-infection may lead to fatal diseases in domestic and small wild cats .
	manualset3
153249	1	408246	13	NULL	NULL	0	NULL	Federal Food	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The Federal Food , Drug , and Cosmetic Act requires the listing of all food ingredients on the label .
	manualset3
153250	2	408246	13	NULL	NULL	0	NULL	Drug 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The Federal Food , Drug , and Cosmetic Act requires the listing of all food ingredients on the label .
	manualset3
153251	3	408246	13	NULL	NULL	0	NULL	Cosmetic Act	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The Federal Food , Drug , and Cosmetic Act requires the listing of all food ingredients on the label .
	manualset3
153252	4	408246	13	NULL	NULL	0	NULL	listing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Federal Food , Drug , and Cosmetic Act requires the listing of all food ingredients on the label .
	manualset3
153253	5	408246	13	NULL	NULL	0	NULL	food ingredients	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The Federal Food , Drug , and Cosmetic Act requires the listing of all food ingredients on the label .
	manualset3
153254	6	408246	13	NULL	NULL	NULL	NULL	label	Thing												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The Federal Food , Drug , and Cosmetic Act requires the listing of all food ingredients on the label .
	manualset3
153255	1	408247	13	NULL	NULL	0	NULL	Fisk splint	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The Fisk splint -- description and assembly .
	manualset3
153256	2	408247	13	NULL	NULL	0	NULL	description	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Fisk splint -- description and assembly .
	manualset3
153257	3	408247	13	NULL	NULL	0	NULL	assembly 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Fisk splint -- description and assembly .
	manualset3
153258	1	408248	13	NULL	NULL	0	NULL	FliG protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The FliG , FliM and FliN proteins form part of recently characterized extended flagellar basal structures , and have been postulated to form a mutually interacting structural complex .
	manualset3
153259	2	408248	13	NULL	NULL	0	NULL	FliM protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The FliG , FliM and FliN proteins form part of recently characterized extended flagellar basal structures , and have been postulated to form a mutually interacting structural complex .
	manualset3
153260	3	408248	13	NULL	NULL	0	NULL	FliN protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The FliG , FliM and FliN proteins form part of recently characterized extended flagellar basal structures , and have been postulated to form a mutually interacting structural complex .
	manualset3
153261	4	408248	13	NULL	NULL	0	NULL	part 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The FliG , FliM and FliN proteins form part of recently characterized extended flagellar basal structures , and have been postulated to form a mutually interacting structural complex .
	manualset3
153262	5	408248	13	NULL	NULL	0	NULL	flagellar basal structures	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The FliG , FliM and FliN proteins form part of recently characterized extended flagellar basal structures , and have been postulated to form a mutually interacting structural complex .
	manualset3
153263	6	408248	13	NULL	NULL	0	NULL	interacting structural complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The FliG , FliM and FliN proteins form part of recently characterized extended flagellar basal structures , and have been postulated to form a mutually interacting structural complex .
	manualset3
153264	1	408249	13	NULL	NULL	0	NULL	G + C content	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The G + C content of the isolate was 34 mol % .
	manualset3
153265	2	408249	13	NULL	NULL	0	NULL	 34 mol %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The G + C content of the isolate was 34 mol % .
	manualset3
153266	1	408250	13	NULL	NULL	0	NULL	method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A rapid and sensitive method for the sequential determination of Cr ( VI ) and Cr ( III ) in water samples based on flame atomic absorption spectrometry with TOA-benzene extraction separation system has been developed .
	manualset3
153267	2	408250	13	NULL	NULL	0	NULL	sequential determination 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A rapid and sensitive method for the sequential determination of Cr ( VI ) and Cr ( III ) in water samples based on flame atomic absorption spectrometry with TOA-benzene extraction separation system has been developed .
	manualset3
153268	3	408250	13	NULL	NULL	0	NULL	Cr ( VI )	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	A rapid and sensitive method for the sequential determination of Cr ( VI ) and Cr ( III ) in water samples based on flame atomic absorption spectrometry with TOA-benzene extraction separation system has been developed .
	manualset3
153269	4	408250	13	NULL	NULL	0	NULL	Cr ( III )	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	A rapid and sensitive method for the sequential determination of Cr ( VI ) and Cr ( III ) in water samples based on flame atomic absorption spectrometry with TOA-benzene extraction separation system has been developed .
	manualset3
153270	5	408250	13	NULL	NULL	0	NULL	water samples	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A rapid and sensitive method for the sequential determination of Cr ( VI ) and Cr ( III ) in water samples based on flame atomic absorption spectrometry with TOA-benzene extraction separation system has been developed .
	manualset3
153271	6	408250	13	NULL	NULL	0	NULL	flame atomic absorption spectrometry 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A rapid and sensitive method for the sequential determination of Cr ( VI ) and Cr ( III ) in water samples based on flame atomic absorption spectrometry with TOA-benzene extraction separation system has been developed .
	manualset3
153272	7	408250	13	NULL	NULL	0	NULL	TOA-benzene extraction separation system 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A rapid and sensitive method for the sequential determination of Cr ( VI ) and Cr ( III ) in water samples based on flame atomic absorption spectrometry with TOA-benzene extraction separation system has been developed .
	manualset3
153273	1	408251	13	NULL	NULL	0	NULL	G protein-coupled receptors ( GPCRs ) 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The G protein-coupled receptors ( GPCRs ) , which form the largest group of transmembrane proteins involved in signal transduction , are major targets of currently available drugs .
	manualset3
153275	3	408251	13	NULL	NULL	0	NULL	group of transmembrane proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The G protein-coupled receptors ( GPCRs ) , which form the largest group of transmembrane proteins involved in signal transduction , are major targets of currently available drugs .
	manualset3
153276	4	408251	13	NULL	NULL	0	NULL	 signal transduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The G protein-coupled receptors ( GPCRs ) , which form the largest group of transmembrane proteins involved in signal transduction , are major targets of currently available drugs .
	manualset3
153277	5	408251	13	NULL	NULL	0	NULL	targets	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The G protein-coupled receptors ( GPCRs ) , which form the largest group of transmembrane proteins involved in signal transduction , are major targets of currently available drugs .
	manualset3
153278	6	408251	13	NULL	NULL	0	NULL	 drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The G protein-coupled receptors ( GPCRs ) , which form the largest group of transmembrane proteins involved in signal transduction , are major targets of currently available drugs .
	manualset3
153279	1	408252	13	NULL	NULL	0	NULL	G protein-coupled receptors ( GPCRs ) 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The G protein-coupled receptors ( GPCRs ) MT ( 1 ) and MT ( 2 ) are capable of parallel or alternate signaling via different Galpha subforms , in particular , Galpha ( i ) ( 2 / ) ( 3 ) and Galpha ( q ) , and via Gbetagamma , as well .
	manualset3
153280	2	408252	13	NULL	NULL	0	NULL	MT ( 1 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The G protein-coupled receptors ( GPCRs ) MT ( 1 ) and MT ( 2 ) are capable of parallel or alternate signaling via different Galpha subforms , in particular , Galpha ( i ) ( 2 / ) ( 3 ) and Galpha ( q ) , and via Gbetagamma , as well .
	manualset3
153281	3	408252	13	NULL	NULL	0	NULL	MT ( 2 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The G protein-coupled receptors ( GPCRs ) MT ( 1 ) and MT ( 2 ) are capable of parallel or alternate signaling via different Galpha subforms , in particular , Galpha ( i ) ( 2 / ) ( 3 ) and Galpha ( q ) , and via Gbetagamma , as well .
	manualset3
153282	4	408252	13	NULL	NULL	0	NULL	 signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The G protein-coupled receptors ( GPCRs ) MT ( 1 ) and MT ( 2 ) are capable of parallel or alternate signaling via different Galpha subforms , in particular , Galpha ( i ) ( 2 / ) ( 3 ) and Galpha ( q ) , and via Gbetagamma , as well .
	manualset3
153283	5	408252	13	NULL	NULL	0	NULL	Galpha subforms 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The G protein-coupled receptors ( GPCRs ) MT ( 1 ) and MT ( 2 ) are capable of parallel or alternate signaling via different Galpha subforms , in particular , Galpha ( i ) ( 2 / ) ( 3 ) and Galpha ( q ) , and via Gbetagamma , as well .
	manualset3
153284	6	408252	13	NULL	NULL	0	NULL	Galpha ( i ) ( 2 / ) ( 3 )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The G protein-coupled receptors ( GPCRs ) MT ( 1 ) and MT ( 2 ) are capable of parallel or alternate signaling via different Galpha subforms , in particular , Galpha ( i ) ( 2 / ) ( 3 ) and Galpha ( q ) , and via Gbetagamma , as well .
	manualset3
153285	7	408252	13	NULL	NULL	0	NULL	Galpha ( q )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The G protein-coupled receptors ( GPCRs ) MT ( 1 ) and MT ( 2 ) are capable of parallel or alternate signaling via different Galpha subforms , in particular , Galpha ( i ) ( 2 / ) ( 3 ) and Galpha ( q ) , and via Gbetagamma , as well .
	manualset3
153286	8	408252	13	NULL	NULL	0	NULL	Gbetagamma	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The G protein-coupled receptors ( GPCRs ) MT ( 1 ) and MT ( 2 ) are capable of parallel or alternate signaling via different Galpha subforms , in particular , Galpha ( i ) ( 2 / ) ( 3 ) and Galpha ( q ) , and via Gbetagamma , as well .
	manualset3
153288	1	408253	13	NULL	NULL	0	NULL	GABA ( B ) R1 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The GABA ( B ) R1 protein was immunohistochemically localized to airway smooth muscle in guinea pig tracheal rings .
	manualset3
153289	2	408253	13	NULL	NULL	0	NULL	airway smooth muscle 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The GABA ( B ) R1 protein was immunohistochemically localized to airway smooth muscle in guinea pig tracheal rings .
	manualset3
153290	3	408253	13	NULL	NULL	0	NULL	guinea pig tracheal rings	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The GABA ( B ) R1 protein was immunohistochemically localized to airway smooth muscle in guinea pig tracheal rings .
	manualset3
153291	1	408254	13	NULL	NULL	0	NULL	 GC-DFHRMS technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The GC-DFHRMS technique provided higher percentage of positive samples and low PCBs median values , due to higher sensitivity and interferences from isobaric ions in the GC-MS technique and is therefore considered as a powerful tool for such assessments in hair specimens .
	manualset3
153292	2	408254	13	NULL	NULL	0	NULL	percentage	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The GC-DFHRMS technique provided higher percentage of positive samples and low PCBs median values , due to higher sensitivity and interferences from isobaric ions in the GC-MS technique and is therefore considered as a powerful tool for such assessments in hair specimens .
	manualset3
153293	3	408254	13	NULL	NULL	0	NULL	positive samples	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The GC-DFHRMS technique provided higher percentage of positive samples and low PCBs median values , due to higher sensitivity and interferences from isobaric ions in the GC-MS technique and is therefore considered as a powerful tool for such assessments in hair specimens .
	manualset3
153294	4	408254	13	NULL	NULL	0	NULL	low PCBs median values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The GC-DFHRMS technique provided higher percentage of positive samples and low PCBs median values , due to higher sensitivity and interferences from isobaric ions in the GC-MS technique and is therefore considered as a powerful tool for such assessments in hair specimens .
	manualset3
153295	5	408254	13	NULL	NULL	0	NULL	sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The GC-DFHRMS technique provided higher percentage of positive samples and low PCBs median values , due to higher sensitivity and interferences from isobaric ions in the GC-MS technique and is therefore considered as a powerful tool for such assessments in hair specimens .
	manualset3
153296	6	408254	13	NULL	NULL	0	NULL	interferences 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The GC-DFHRMS technique provided higher percentage of positive samples and low PCBs median values , due to higher sensitivity and interferences from isobaric ions in the GC-MS technique and is therefore considered as a powerful tool for such assessments in hair specimens .
	manualset3
153297	7	408254	13	NULL	NULL	0	NULL	isobaric ions 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The GC-DFHRMS technique provided higher percentage of positive samples and low PCBs median values , due to higher sensitivity and interferences from isobaric ions in the GC-MS technique and is therefore considered as a powerful tool for such assessments in hair specimens .
	manualset3
153298	8	408254	13	NULL	NULL	0	NULL	GC-MS technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The GC-DFHRMS technique provided higher percentage of positive samples and low PCBs median values , due to higher sensitivity and interferences from isobaric ions in the GC-MS technique and is therefore considered as a powerful tool for such assessments in hair specimens .
	manualset3
153299	9	408254	13	NULL	NULL	0	NULL	tool 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The GC-DFHRMS technique provided higher percentage of positive samples and low PCBs median values , due to higher sensitivity and interferences from isobaric ions in the GC-MS technique and is therefore considered as a powerful tool for such assessments in hair specimens .
	manualset3
153300	10	408254	13	NULL	NULL	0	NULL	assessments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The GC-DFHRMS technique provided higher percentage of positive samples and low PCBs median values , due to higher sensitivity and interferences from isobaric ions in the GC-MS technique and is therefore considered as a powerful tool for such assessments in hair specimens .
	manualset3
153301	11	408254	13	NULL	NULL	0	NULL	hair specimens 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The GC-DFHRMS technique provided higher percentage of positive samples and low PCBs median values , due to higher sensitivity and interferences from isobaric ions in the GC-MS technique and is therefore considered as a powerful tool for such assessments in hair specimens .
	manualset3
153302	1	408255	13	NULL	NULL	0	NULL	 GM3 content	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The GM3 and GD3 content of the meningiomas belonging to the 2 groups revealed a significant correlation between amount and reciprocal ratio of these 2 gangliosides and cytogenetic data .
	manualset3
153303	2	408255	13	NULL	NULL	0	NULL	GD3 content 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The GM3 and GD3 content of the meningiomas belonging to the 2 groups revealed a significant correlation between amount and reciprocal ratio of these 2 gangliosides and cytogenetic data .
	manualset3
153304	3	408255	13	NULL	NULL	0	NULL	meningiomas 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The GM3 and GD3 content of the meningiomas belonging to the 2 groups revealed a significant correlation between amount and reciprocal ratio of these 2 gangliosides and cytogenetic data .
	manualset3
153305	4	408255	13	NULL	NULL	0	NULL	2 groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The GM3 and GD3 content of the meningiomas belonging to the 2 groups revealed a significant correlation between amount and reciprocal ratio of these 2 gangliosides and cytogenetic data .
	manualset3
153306	5	408255	13	NULL	NULL	0	NULL	correlation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The GM3 and GD3 content of the meningiomas belonging to the 2 groups revealed a significant correlation between amount and reciprocal ratio of these 2 gangliosides and cytogenetic data .
	manualset3
153307	6	408255	13	NULL	NULL	0	NULL	amount	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The GM3 and GD3 content of the meningiomas belonging to the 2 groups revealed a significant correlation between amount and reciprocal ratio of these 2 gangliosides and cytogenetic data .
	manualset3
153308	7	408255	13	NULL	NULL	0	NULL	reciprocal ratio	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The GM3 and GD3 content of the meningiomas belonging to the 2 groups revealed a significant correlation between amount and reciprocal ratio of these 2 gangliosides and cytogenetic data .
	manualset3
153309	8	408255	13	NULL	NULL	0	NULL	2 gangliosides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The GM3 and GD3 content of the meningiomas belonging to the 2 groups revealed a significant correlation between amount and reciprocal ratio of these 2 gangliosides and cytogenetic data .
	manualset3
153310	9	408255	13	NULL	NULL	0	NULL	cytogenetic data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The GM3 and GD3 content of the meningiomas belonging to the 2 groups revealed a significant correlation between amount and reciprocal ratio of these 2 gangliosides and cytogenetic data .
	manualset3
153311	1	408256	13	NULL	NULL	0	NULL	GP antagonist-2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The GP antagonist-2 , which blocks Gs , prevented the inhibitory effect of Abeta on the glucose uptake .
	manualset3
153313	3	408256	13	NULL	NULL	0	NULL	Gs	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The GP antagonist-2 , which blocks Gs , prevented the inhibitory effect of Abeta on the glucose uptake .
	manualset3
153314	4	408256	13	NULL	NULL	0	NULL	inhibitory effect 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The GP antagonist-2 , which blocks Gs , prevented the inhibitory effect of Abeta on the glucose uptake .
	manualset3
153315	5	408256	13	NULL	NULL	0	NULL	Abeta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The GP antagonist-2 , which blocks Gs , prevented the inhibitory effect of Abeta on the glucose uptake .
	manualset3
153316	6	408256	13	NULL	NULL	0	NULL	glucose uptake	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The GP antagonist-2 , which blocks Gs , prevented the inhibitory effect of Abeta on the glucose uptake .
	manualset3
153317	1	408257	13	NULL	NULL	0	NULL	GP perspective	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The GP perspective : problems experienced in providing diabetes care in UK general practice .
	manualset3
153318	2	408257	13	NULL	NULL	0	NULL	problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The GP perspective : problems experienced in providing diabetes care in UK general practice .
	manualset3
153319	3	408257	13	NULL	NULL	0	NULL	diabetes care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The GP perspective : problems experienced in providing diabetes care in UK general practice .
	manualset3
153320	4	408257	13	NULL	NULL	0	NULL	UK	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The GP perspective : problems experienced in providing diabetes care in UK general practice .
	manualset3
153321	5	408257	13	NULL	NULL	0	NULL	general practice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The GP perspective : problems experienced in providing diabetes care in UK general practice .
	manualset3
153322	1	408258	13	NULL	NULL	0	NULL	GPP 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The GPP is a coaxial arrangement with inner and outer electrodes and utilizes a corona discharge to electrically charge the particles and a strong electric field to remove them from the sample flow .
	manualset3
153323	2	408258	13	NULL	NULL	0	NULL	coaxial arrangement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The GPP is a coaxial arrangement with inner and outer electrodes and utilizes a corona discharge to electrically charge the particles and a strong electric field to remove them from the sample flow .
	manualset3
153324	3	408258	13	NULL	NULL	0	NULL	 inner electrodes 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The GPP is a coaxial arrangement with inner and outer electrodes and utilizes a corona discharge to electrically charge the particles and a strong electric field to remove them from the sample flow .
	manualset3
153325	4	408258	13	NULL	NULL	0	NULL	outer electrodes	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The GPP is a coaxial arrangement with inner and outer electrodes and utilizes a corona discharge to electrically charge the particles and a strong electric field to remove them from the sample flow .
	manualset3
153326	5	408258	13	NULL	NULL	0	NULL	corona discharge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The GPP is a coaxial arrangement with inner and outer electrodes and utilizes a corona discharge to electrically charge the particles and a strong electric field to remove them from the sample flow .
	manualset3
153327	6	408258	13	NULL	NULL	0	NULL	particles	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The GPP is a coaxial arrangement with inner and outer electrodes and utilizes a corona discharge to electrically charge the particles and a strong electric field to remove them from the sample flow .
	manualset3
153328	7	408258	13	NULL	NULL	0	NULL	electric field	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The GPP is a coaxial arrangement with inner and outer electrodes and utilizes a corona discharge to electrically charge the particles and a strong electric field to remove them from the sample flow .
	manualset3
153329	8	408258	13	NULL	NULL	0	NULL	sample flow	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The GPP is a coaxial arrangement with inner and outer electrodes and utilizes a corona discharge to electrically charge the particles and a strong electric field to remove them from the sample flow .
	manualset3
153330	1	408259	13	NULL	NULL	0	NULL	GPi FPs 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The GPi FPs showed temporal correlation with EMG-recorded rectus abdominis potentials .
	manualset3
153331	2	408259	13	NULL	NULL	0	NULL	temporal correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The GPi FPs showed temporal correlation with EMG-recorded rectus abdominis potentials .
	manualset3
153332	3	408259	13	NULL	NULL	0	NULL	EMG-recorded rectus abdominis potentials	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The GPi FPs showed temporal correlation with EMG-recorded rectus abdominis potentials .
	manualset3
153333	1	408260	13	NULL	NULL	0	NULL	oxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A rapid oxidation of NADH suddenly began at the end of the induction phase and the oxidation continued at a relatively constant rate .
	manualset3
153334	2	408260	13	NULL	NULL	0	NULL	NADH 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A rapid oxidation of NADH suddenly began at the end of the induction phase and the oxidation continued at a relatively constant rate .
	manualset3
153335	3	408260	13	NULL	NULL	0	NULL	end 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A rapid oxidation of NADH suddenly began at the end of the induction phase and the oxidation continued at a relatively constant rate .
	manualset3
153336	4	408260	13	NULL	NULL	0	NULL	induction phase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A rapid oxidation of NADH suddenly began at the end of the induction phase and the oxidation continued at a relatively constant rate .
	manualset3
153337	5	408260	13	NULL	NULL	0	NULL	oxidation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A rapid oxidation of NADH suddenly began at the end of the induction phase and the oxidation continued at a relatively constant rate .
	manualset3
153338	6	408260	13	NULL	NULL	0	NULL	constant rate 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A rapid oxidation of NADH suddenly began at the end of the induction phase and the oxidation continued at a relatively constant rate .
	manualset3
153339	1	408261	13	NULL	NULL	0	NULL	GSTP1 Val allele	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The GSTP1 Val allele was shown to be a risk factor for NAFLD ( OR = 1.739 , 95 % CI = 1.089-2 .777 , p = 0.024 ) .
	manualset3
153340	2	408261	13	NULL	NULL	0	NULL	risk factor 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The GSTP1 Val allele was shown to be a risk factor for NAFLD ( OR = 1.739 , 95 % CI = 1.089-2 .777 , p = 0.024 ) .
	manualset3
153341	3	408261	13	NULL	NULL	0	NULL	NAFLD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The GSTP1 Val allele was shown to be a risk factor for NAFLD ( OR = 1.739 , 95 % CI = 1.089-2 .777 , p = 0.024 ) .
	manualset3
153342	4	408261	13	NULL	NULL	0	NULL	 OR = 1.739 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The GSTP1 Val allele was shown to be a risk factor for NAFLD ( OR = 1.739 , 95 % CI = 1.089-2 .777 , p = 0.024 ) .
	manualset3
153343	5	408261	13	NULL	NULL	0	NULL	95 % CI = 1.089-2 .777	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The GSTP1 Val allele was shown to be a risk factor for NAFLD ( OR = 1.739 , 95 % CI = 1.089-2 .777 , p = 0.024 ) .
	manualset3
153344	6	408261	13	NULL	NULL	0	NULL	p = 0.024	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The GSTP1 Val allele was shown to be a risk factor for NAFLD ( OR = 1.739 , 95 % CI = 1.089-2 .777 , p = 0.024 ) .
	manualset3
153345	1	408262	13	NULL	NULL	0	NULL	 GTP-bound conformation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The GTP-bound conformation is biologically active and promotes a cellular function , such as signal transduction , cytoskeleton organization , protein synthesis/translocation , or a membrane budding/fusion event .
	manualset3
153346	2	408262	13	NULL	NULL	0	NULL	cellular function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The GTP-bound conformation is biologically active and promotes a cellular function , such as signal transduction , cytoskeleton organization , protein synthesis/translocation , or a membrane budding/fusion event .
	manualset3
153347	3	408262	13	NULL	NULL	0	NULL	 signal transduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The GTP-bound conformation is biologically active and promotes a cellular function , such as signal transduction , cytoskeleton organization , protein synthesis/translocation , or a membrane budding/fusion event .
	manualset3
153348	4	408262	13	NULL	NULL	0	NULL	cytoskeleton organization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The GTP-bound conformation is biologically active and promotes a cellular function , such as signal transduction , cytoskeleton organization , protein synthesis/translocation , or a membrane budding/fusion event .
	manualset3
153349	5	408262	13	NULL	NULL	0	NULL	protein synthesis/translocation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The GTP-bound conformation is biologically active and promotes a cellular function , such as signal transduction , cytoskeleton organization , protein synthesis/translocation , or a membrane budding/fusion event .
	manualset3
153350	6	408262	13	NULL	NULL	0	NULL	membrane budding/fusion event	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The GTP-bound conformation is biologically active and promotes a cellular function , such as signal transduction , cytoskeleton organization , protein synthesis/translocation , or a membrane budding/fusion event .
	manualset3
153352	1	408263	13	NULL	NULL	NULL	NULL	GlucoWatch biographer 	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The GlucoWatch ( Cygnus , Inc , Redwood City , CA , USA ) biographer provides automatic , frequent and noninvasive blood glucose measurements for up to 12 h. The device extracts glucose through intact skin where it is measured by an amperometric biosensor .
	manualset3
153353	2	408263	13	NULL	NULL	0	NULL	Cygnus , Inc	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The GlucoWatch ( Cygnus , Inc , Redwood City , CA , USA ) biographer provides automatic , frequent and noninvasive blood glucose measurements for up to 12 h. The device extracts glucose through intact skin where it is measured by an amperometric biosensor .
	manualset3
153354	3	408263	13	NULL	NULL	0	NULL	Redwood City	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The GlucoWatch ( Cygnus , Inc , Redwood City , CA , USA ) biographer provides automatic , frequent and noninvasive blood glucose measurements for up to 12 h. The device extracts glucose through intact skin where it is measured by an amperometric biosensor .
	manualset3
153355	4	408263	13	NULL	NULL	0	NULL	CA	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The GlucoWatch ( Cygnus , Inc , Redwood City , CA , USA ) biographer provides automatic , frequent and noninvasive blood glucose measurements for up to 12 h. The device extracts glucose through intact skin where it is measured by an amperometric biosensor .
	manualset3
153356	5	408263	13	NULL	NULL	0	NULL	USA	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The GlucoWatch ( Cygnus , Inc , Redwood City , CA , USA ) biographer provides automatic , frequent and noninvasive blood glucose measurements for up to 12 h. The device extracts glucose through intact skin where it is measured by an amperometric biosensor .
	manualset3
153357	6	408263	13	NULL	NULL	0	NULL	blood glucose measurements 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The GlucoWatch ( Cygnus , Inc , Redwood City , CA , USA ) biographer provides automatic , frequent and noninvasive blood glucose measurements for up to 12 h. The device extracts glucose through intact skin where it is measured by an amperometric biosensor .
	manualset3
153358	7	408263	13	NULL	NULL	0	NULL	12 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The GlucoWatch ( Cygnus , Inc , Redwood City , CA , USA ) biographer provides automatic , frequent and noninvasive blood glucose measurements for up to 12 h. The device extracts glucose through intact skin where it is measured by an amperometric biosensor .
	manualset3
153359	8	408263	13	NULL	NULL	0	NULL	device 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The GlucoWatch ( Cygnus , Inc , Redwood City , CA , USA ) biographer provides automatic , frequent and noninvasive blood glucose measurements for up to 12 h. The device extracts glucose through intact skin where it is measured by an amperometric biosensor .
	manualset3
153361	10	408263	13	NULL	NULL	0	NULL	glucose	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The GlucoWatch ( Cygnus , Inc , Redwood City , CA , USA ) biographer provides automatic , frequent and noninvasive blood glucose measurements for up to 12 h. The device extracts glucose through intact skin where it is measured by an amperometric biosensor .
	manualset3
153362	11	408263	13	NULL	NULL	0	NULL	skin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The GlucoWatch ( Cygnus , Inc , Redwood City , CA , USA ) biographer provides automatic , frequent and noninvasive blood glucose measurements for up to 12 h. The device extracts glucose through intact skin where it is measured by an amperometric biosensor .
	manualset3
153363	12	408263	13	NULL	NULL	0	NULL	amperometric biosensor	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The GlucoWatch ( Cygnus , Inc , Redwood City , CA , USA ) biographer provides automatic , frequent and noninvasive blood glucose measurements for up to 12 h. The device extracts glucose through intact skin where it is measured by an amperometric biosensor .
	manualset3
153364	1	408264	13	NULL	NULL	0	NULL	Glut-1 staining index	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Glut-1 staining index in primary HNSCCAs was significantly lower than that in recurrent HNSCCAs ( P = 0.03 ) , and the index of better-differentiated tumors lower than that of poorly-differentiated tumors ( P = 0.02 ) .
	manualset3
153365	2	408264	13	NULL	NULL	0	NULL	primary HNSCCAs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The Glut-1 staining index in primary HNSCCAs was significantly lower than that in recurrent HNSCCAs ( P = 0.03 ) , and the index of better-differentiated tumors lower than that of poorly-differentiated tumors ( P = 0.02 ) .
	manualset3
153366	3	408264	13	NULL	NULL	NULL	NULL	 recurrent HNSCCAs 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The Glut-1 staining index in primary HNSCCAs was significantly lower than that in recurrent HNSCCAs ( P = 0.03 ) , and the index of better-differentiated tumors lower than that of poorly-differentiated tumors ( P = 0.02 ) .
	manualset3
153367	4	408264	13	NULL	NULL	0	NULL	P = 0.03	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Glut-1 staining index in primary HNSCCAs was significantly lower than that in recurrent HNSCCAs ( P = 0.03 ) , and the index of better-differentiated tumors lower than that of poorly-differentiated tumors ( P = 0.02 ) .
	manualset3
153368	5	408264	13	NULL	NULL	0	NULL	 index 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Glut-1 staining index in primary HNSCCAs was significantly lower than that in recurrent HNSCCAs ( P = 0.03 ) , and the index of better-differentiated tumors lower than that of poorly-differentiated tumors ( P = 0.02 ) .
	manualset3
153369	6	408264	13	NULL	NULL	NULL	NULL	 better-differentiated tumors 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The Glut-1 staining index in primary HNSCCAs was significantly lower than that in recurrent HNSCCAs ( P = 0.03 ) , and the index of better-differentiated tumors lower than that of poorly-differentiated tumors ( P = 0.02 ) .
	manualset3
153370	7	408264	13	NULL	NULL	0	NULL	poorly-differentiated tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Glut-1 staining index in primary HNSCCAs was significantly lower than that in recurrent HNSCCAs ( P = 0.03 ) , and the index of better-differentiated tumors lower than that of poorly-differentiated tumors ( P = 0.02 ) .
	manualset3
153371	8	408264	13	NULL	NULL	0	NULL	P = 0.02	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Glut-1 staining index in primary HNSCCAs was significantly lower than that in recurrent HNSCCAs ( P = 0.03 ) , and the index of better-differentiated tumors lower than that of poorly-differentiated tumors ( P = 0.02 ) .
	manualset3
153372	1	408265	13	NULL	NULL	0	NULL	GnRH 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The GnRH was administered approximately 30 h after the time of norgestomet implant removal ( or 58 h after the second PGF2 alpha injection ) .
	manualset3
153373	2	408265	13	NULL	NULL	0	NULL	30 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The GnRH was administered approximately 30 h after the time of norgestomet implant removal ( or 58 h after the second PGF2 alpha injection ) .
	manualset3
153374	3	408265	13	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The GnRH was administered approximately 30 h after the time of norgestomet implant removal ( or 58 h after the second PGF2 alpha injection ) .
	manualset3
153375	4	408265	13	NULL	NULL	0	NULL	norgestomet implant removal 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The GnRH was administered approximately 30 h after the time of norgestomet implant removal ( or 58 h after the second PGF2 alpha injection ) .
	manualset3
153376	5	408265	13	NULL	NULL	0	NULL	58 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The GnRH was administered approximately 30 h after the time of norgestomet implant removal ( or 58 h after the second PGF2 alpha injection ) .
	manualset3
153377	6	408265	13	NULL	NULL	0	NULL	second PGF2 alpha injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The GnRH was administered approximately 30 h after the time of norgestomet implant removal ( or 58 h after the second PGF2 alpha injection ) .
	manualset3
153378	1	408266	13	NULL	NULL	0	NULL	Guinea pig	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The Guinea pig is a potentially interesting alternative small animal model for the study of the neuroendocrine regulation of reproduction .
	manualset3
153379	2	408266	13	NULL	NULL	0	NULL	alternative small animal model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The Guinea pig is a potentially interesting alternative small animal model for the study of the neuroendocrine regulation of reproduction .
	manualset3
153380	3	408266	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Guinea pig is a potentially interesting alternative small animal model for the study of the neuroendocrine regulation of reproduction .
	manualset3
153381	4	408266	13	NULL	NULL	0	NULL	neuroendocrine regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Guinea pig is a potentially interesting alternative small animal model for the study of the neuroendocrine regulation of reproduction .
	manualset3
153382	5	408266	13	NULL	NULL	0	NULL	reproduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Guinea pig is a potentially interesting alternative small animal model for the study of the neuroendocrine regulation of reproduction .
	manualset3
153383	1	408267	13	NULL	NULL	0	NULL	HIV RT 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The HIV RT and Protease Sequence Database is an on-line relational database that catalogues evolutionary and drug-related human immunodeficiency virus reverse transcriptase ( RT ) and protease sequence variation ( http : //hivdb.stanford.edu ) .
	manualset3
153384	2	408267	13	NULL	NULL	0	NULL	Protease Sequence Database 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The HIV RT and Protease Sequence Database is an on-line relational database that catalogues evolutionary and drug-related human immunodeficiency virus reverse transcriptase ( RT ) and protease sequence variation ( http : //hivdb.stanford.edu ) .
	manualset3
153385	3	408267	13	NULL	NULL	0	NULL	on-line relational database 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The HIV RT and Protease Sequence Database is an on-line relational database that catalogues evolutionary and drug-related human immunodeficiency virus reverse transcriptase ( RT ) and protease sequence variation ( http : //hivdb.stanford.edu ) .
	manualset3
153386	4	408267	13	NULL	NULL	0	NULL	catalogues	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The HIV RT and Protease Sequence Database is an on-line relational database that catalogues evolutionary and drug-related human immunodeficiency virus reverse transcriptase ( RT ) and protease sequence variation ( http : //hivdb.stanford.edu ) .
	manualset3
153387	5	408267	13	NULL	NULL	0	NULL	drug-related human immunodeficiency virus reverse transcriptase ( RT )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The HIV RT and Protease Sequence Database is an on-line relational database that catalogues evolutionary and drug-related human immunodeficiency virus reverse transcriptase ( RT ) and protease sequence variation ( http : //hivdb.stanford.edu ) .
	manualset3
153388	6	408267	13	NULL	NULL	0	NULL	protease sequence variation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The HIV RT and Protease Sequence Database is an on-line relational database that catalogues evolutionary and drug-related human immunodeficiency virus reverse transcriptase ( RT ) and protease sequence variation ( http : //hivdb.stanford.edu ) .
	manualset3
153389	7	408267	13	NULL	NULL	0	NULL	http : //hivdb.stanford.edu	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The HIV RT and Protease Sequence Database is an on-line relational database that catalogues evolutionary and drug-related human immunodeficiency virus reverse transcriptase ( RT ) and protease sequence variation ( http : //hivdb.stanford.edu ) .
	manualset3
153390	1	408268	13	NULL	NULL	0	NULL	serious condition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A rare , but serious condition ) .
	manualset3
153391	1	408269	13	NULL	NULL	0	NULL	 HIV protein Vpu 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The HIV protein Vpu antagonizes this host defense .
	manualset3
153392	2	408269	13	NULL	NULL	0	NULL	host defense	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The HIV protein Vpu antagonizes this host defense .
	manualset3
153393	1	408270	13	NULL	NULL	0	NULL	HLA-DRI5 tissue type 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The HLA-DRI5 tissue type was present in 47 % ( 43 % ) .
	manualset3
153394	2	408270	13	NULL	NULL	0	NULL	47 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The HLA-DRI5 tissue type was present in 47 % ( 43 % ) .
	manualset3
153395	3	408270	13	NULL	NULL	0	NULL	43 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The HLA-DRI5 tissue type was present in 47 % ( 43 % ) .
	manualset3
153396	1	408271	13	NULL	NULL	0	NULL	HMG box	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The HMG box itself as a DNA-binding motif may have the basic function of inducing curvature , resulting in the apparent DNA bending in the DNA cyclization assay , but not of abruptly kinking DNA .
	manualset3
153397	2	408271	13	NULL	NULL	0	NULL	DNA-binding motif 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The HMG box itself as a DNA-binding motif may have the basic function of inducing curvature , resulting in the apparent DNA bending in the DNA cyclization assay , but not of abruptly kinking DNA .
	manualset3
153398	3	408271	13	NULL	NULL	0	NULL	function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The HMG box itself as a DNA-binding motif may have the basic function of inducing curvature , resulting in the apparent DNA bending in the DNA cyclization assay , but not of abruptly kinking DNA .
	manualset3
153399	4	408271	13	NULL	NULL	0	NULL	curvature	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The HMG box itself as a DNA-binding motif may have the basic function of inducing curvature , resulting in the apparent DNA bending in the DNA cyclization assay , but not of abruptly kinking DNA .
	manualset3
153400	5	408271	13	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The HMG box itself as a DNA-binding motif may have the basic function of inducing curvature , resulting in the apparent DNA bending in the DNA cyclization assay , but not of abruptly kinking DNA .
	manualset3
153401	6	408271	13	NULL	NULL	0	NULL	DNA cyclization assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The HMG box itself as a DNA-binding motif may have the basic function of inducing curvature , resulting in the apparent DNA bending in the DNA cyclization assay , but not of abruptly kinking DNA .
	manualset3
153402	7	408271	13	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The HMG box itself as a DNA-binding motif may have the basic function of inducing curvature , resulting in the apparent DNA bending in the DNA cyclization assay , but not of abruptly kinking DNA .
	manualset3
153403	1	408272	13	NULL	NULL	0	NULL	HSA viscosities 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The HSA viscosities determined at 200 s ( -1 ) were 1.1 , 4.2 and 6.0 dyn x cm ( -2 ) , respectively .
	manualset3
153404	2	408272	13	NULL	NULL	0	NULL	200 s ( -1 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The HSA viscosities determined at 200 s ( -1 ) were 1.1 , 4.2 and 6.0 dyn x cm ( -2 ) , respectively .
	manualset3
153405	3	408272	13	NULL	NULL	0	NULL	1.1 dyn x cm ( -2 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The HSA viscosities determined at 200 s ( -1 ) were 1.1 , 4.2 and 6.0 dyn x cm ( -2 ) , respectively .
	manualset3
153406	4	408272	13	NULL	NULL	0	NULL	4.2 dyn x cm ( -2 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The HSA viscosities determined at 200 s ( -1 ) were 1.1 , 4.2 and 6.0 dyn x cm ( -2 ) , respectively .
	manualset3
153407	5	408272	13	NULL	NULL	0	NULL	6.0 dyn x cm ( -2 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The HSA viscosities determined at 200 s ( -1 ) were 1.1 , 4.2 and 6.0 dyn x cm ( -2 ) , respectively .
	manualset3
153408	1	408273	13	NULL	NULL	0	NULL	HiNF-P/p220 ( NPAT ) complex 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The HiNF-P/p220 ( NPAT ) complex controls multiple H4 genes in established human cell lines and is critical for cell proliferation .
	manualset3
153409	2	408273	13	NULL	NULL	0	NULL	controls	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The HiNF-P/p220 ( NPAT ) complex controls multiple H4 genes in established human cell lines and is critical for cell proliferation .
	manualset3
153410	3	408273	13	NULL	NULL	0	NULL	multiple H4 genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The HiNF-P/p220 ( NPAT ) complex controls multiple H4 genes in established human cell lines and is critical for cell proliferation .
	manualset3
153411	4	408273	13	NULL	NULL	0	NULL	human cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The HiNF-P/p220 ( NPAT ) complex controls multiple H4 genes in established human cell lines and is critical for cell proliferation .
	manualset3
153412	5	408273	13	NULL	NULL	0	NULL	cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The HiNF-P/p220 ( NPAT ) complex controls multiple H4 genes in established human cell lines and is critical for cell proliferation .
	manualset3
153413	1	408274	13	NULL	NULL	0	NULL	Hirase method	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The Hirase method has proven to be a simple and reliable surgical technique for fingertip re-attachment .
	manualset3
153414	2	408274	13	NULL	NULL	0	NULL	surgical technique	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The Hirase method has proven to be a simple and reliable surgical technique for fingertip re-attachment .
	manualset3
153415	3	408274	13	NULL	NULL	0	NULL	fingertip re-attachment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The Hirase method has proven to be a simple and reliable surgical technique for fingertip re-attachment .
	manualset3
153416	1	408275	13	NULL	NULL	0	NULL	Hsp90 inhibitor 17DMAG	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The Hsp90 inhibitor 17DMAG ( 17-dimethylaminoethylamino-17-demethoxygeldanamycin ) is undergoing clinical trials as an antitumor drug .
	manualset3
153417	2	408275	13	NULL	NULL	0	NULL	17-dimethylaminoethylamino-17-demethoxygeldanamycin 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The Hsp90 inhibitor 17DMAG ( 17-dimethylaminoethylamino-17-demethoxygeldanamycin ) is undergoing clinical trials as an antitumor drug .
	manualset3
153418	3	408275	13	NULL	NULL	0	NULL	clinical trials	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Hsp90 inhibitor 17DMAG ( 17-dimethylaminoethylamino-17-demethoxygeldanamycin ) is undergoing clinical trials as an antitumor drug .
	manualset3
153420	4	408275	13	NULL	NULL	0	NULL	antitumor drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The Hsp90 inhibitor 17DMAG ( 17-dimethylaminoethylamino-17-demethoxygeldanamycin ) is undergoing clinical trials as an antitumor drug .
	manualset3
153421	1	408276	13	NULL	NULL	0	NULL	 Hsp90 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The Hsp90 protein from the parasite Plasmodium falciparum , the causative agent of malaria , is critical for this organism 's survival ; the anti-Hsp90 drug geldanamycin is toxic to P. falciparum growth .
	manualset3
153422	2	408276	13	NULL	NULL	0	NULL	parasite Plasmodium falciparum 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The Hsp90 protein from the parasite Plasmodium falciparum , the causative agent of malaria , is critical for this organism 's survival ; the anti-Hsp90 drug geldanamycin is toxic to P. falciparum growth .
	manualset3
153423	3	408276	13	NULL	NULL	0	NULL	causative agent 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The Hsp90 protein from the parasite Plasmodium falciparum , the causative agent of malaria , is critical for this organism 's survival ; the anti-Hsp90 drug geldanamycin is toxic to P. falciparum growth .
	manualset3
153424	4	408276	13	NULL	NULL	0	NULL	malaria	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The Hsp90 protein from the parasite Plasmodium falciparum , the causative agent of malaria , is critical for this organism 's survival ; the anti-Hsp90 drug geldanamycin is toxic to P. falciparum growth .
	manualset3
153425	5	408276	13	NULL	NULL	0	NULL	organism 's survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Hsp90 protein from the parasite Plasmodium falciparum , the causative agent of malaria , is critical for this organism 's survival ; the anti-Hsp90 drug geldanamycin is toxic to P. falciparum growth .
	manualset3
153426	6	408276	13	NULL	NULL	0	NULL	anti-Hsp90 drug geldanamycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The Hsp90 protein from the parasite Plasmodium falciparum , the causative agent of malaria , is critical for this organism 's survival ; the anti-Hsp90 drug geldanamycin is toxic to P. falciparum growth .
	manualset3
153427	7	408276	13	NULL	NULL	0	NULL	P. falciparum growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Hsp90 protein from the parasite Plasmodium falciparum , the causative agent of malaria , is critical for this organism 's survival ; the anti-Hsp90 drug geldanamycin is toxic to P. falciparum growth .
	manualset3
153428	1	408277	13	NULL	NULL	0	NULL	I+III 2 supercomplex 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The I+III 2 supercomplex was found to be a rigid structure which did not break down into subcomplexes at the interface between the hydrophilic and the hydrophobic arms of complex I. The complex I moiety of the supercomplex appears to be only of `` type I '' .
	manualset3
153429	2	408277	13	NULL	NULL	0	NULL	rigid structure	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The I+III 2 supercomplex was found to be a rigid structure which did not break down into subcomplexes at the interface between the hydrophilic and the hydrophobic arms of complex I. The complex I moiety of the supercomplex appears to be only of `` type I '' .
	manualset3
153430	3	408277	13	NULL	NULL	0	NULL	subcomplexes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The I+III 2 supercomplex was found to be a rigid structure which did not break down into subcomplexes at the interface between the hydrophilic and the hydrophobic arms of complex I. The complex I moiety of the supercomplex appears to be only of `` type I '' .
	manualset3
153431	4	408277	13	NULL	NULL	0	NULL	 interface 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The I+III 2 supercomplex was found to be a rigid structure which did not break down into subcomplexes at the interface between the hydrophilic and the hydrophobic arms of complex I. The complex I moiety of the supercomplex appears to be only of `` type I '' .
	manualset3
153432	5	408277	13	NULL	NULL	0	NULL	hydrophilic arms of complex I	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The I+III 2 supercomplex was found to be a rigid structure which did not break down into subcomplexes at the interface between the hydrophilic and the hydrophobic arms of complex I. The complex I moiety of the supercomplex appears to be only of `` type I '' .
	manualset3
153433	6	408277	13	NULL	NULL	0	NULL	hydrophobic arms of complex I	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The I+III 2 supercomplex was found to be a rigid structure which did not break down into subcomplexes at the interface between the hydrophilic and the hydrophobic arms of complex I. The complex I moiety of the supercomplex appears to be only of `` type I '' .
	manualset3
153434	7	408277	13	NULL	NULL	0	NULL	complex I moiety	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The I+III 2 supercomplex was found to be a rigid structure which did not break down into subcomplexes at the interface between the hydrophilic and the hydrophobic arms of complex I. The complex I moiety of the supercomplex appears to be only of `` type I '' .
	manualset3
153435	8	408277	13	NULL	NULL	0	NULL	supercomplex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The I+III 2 supercomplex was found to be a rigid structure which did not break down into subcomplexes at the interface between the hydrophilic and the hydrophobic arms of complex I. The complex I moiety of the supercomplex appears to be only of `` type I '' .
	manualset3
153436	9	408277	13	NULL	NULL	0	NULL	type I	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The I+III 2 supercomplex was found to be a rigid structure which did not break down into subcomplexes at the interface between the hydrophilic and the hydrophobic arms of complex I. The complex I moiety of the supercomplex appears to be only of `` type I '' .
	manualset3
153438	1	408278	13	NULL	NULL	0	NULL	IADSA	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The IADSA has been performed as road mapping prior to therapy .
	manualset3
153439	2	408278	13	NULL	NULL	0	NULL	road mapping	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The IADSA has been performed as road mapping prior to therapy .
	manualset3
153440	3	408278	13	NULL	NULL	0	NULL	therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The IADSA has been performed as road mapping prior to therapy .
	manualset3
153441	1	408279	13	NULL	NULL	0	NULL	IC ( 50 ) values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The IC ( 50 ) values for different inhibitors of the Tat/TAR complex both with wt-TAR and mutants have been determined .
	manualset3
153442	2	408279	13	NULL	NULL	0	NULL	inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The IC ( 50 ) values for different inhibitors of the Tat/TAR complex both with wt-TAR and mutants have been determined .
	manualset3
153443	3	408279	13	NULL	NULL	0	NULL	Tat/TAR complex 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The IC ( 50 ) values for different inhibitors of the Tat/TAR complex both with wt-TAR and mutants have been determined .
	manualset3
153444	4	408279	13	NULL	NULL	NULL	NULL	wt-TAR 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The IC ( 50 ) values for different inhibitors of the Tat/TAR complex both with wt-TAR and mutants have been determined .
	manualset3
153445	5	408279	13	NULL	NULL	NULL	NULL	mutants	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The IC ( 50 ) values for different inhibitors of the Tat/TAR complex both with wt-TAR and mutants have been determined .
	manualset3
153446	1	408280	13	NULL	NULL	0	NULL	ICNP case study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ICNP case study demonstrated both the applicability of the TQI model and the appropriateness of the criteria identified in the TQI model : openness and responsiveness , clarity and reproducibility , understandability , accessibility and usability , interoperability , and quality of documentation .
	manualset3
153447	2	408280	13	NULL	NULL	0	NULL	applicability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ICNP case study demonstrated both the applicability of the TQI model and the appropriateness of the criteria identified in the TQI model : openness and responsiveness , clarity and reproducibility , understandability , accessibility and usability , interoperability , and quality of documentation .
	manualset3
153448	3	408280	13	NULL	NULL	0	NULL	TQI model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The ICNP case study demonstrated both the applicability of the TQI model and the appropriateness of the criteria identified in the TQI model : openness and responsiveness , clarity and reproducibility , understandability , accessibility and usability , interoperability , and quality of documentation .
	manualset3
153449	4	408280	13	NULL	NULL	0	NULL	appropriateness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ICNP case study demonstrated both the applicability of the TQI model and the appropriateness of the criteria identified in the TQI model : openness and responsiveness , clarity and reproducibility , understandability , accessibility and usability , interoperability , and quality of documentation .
	manualset3
153450	5	408280	13	NULL	NULL	0	NULL	criteria	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ICNP case study demonstrated both the applicability of the TQI model and the appropriateness of the criteria identified in the TQI model : openness and responsiveness , clarity and reproducibility , understandability , accessibility and usability , interoperability , and quality of documentation .
	manualset3
153451	6	408280	13	NULL	NULL	0	NULL	TQI model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The ICNP case study demonstrated both the applicability of the TQI model and the appropriateness of the criteria identified in the TQI model : openness and responsiveness , clarity and reproducibility , understandability , accessibility and usability , interoperability , and quality of documentation .
	manualset3
153452	7	408280	13	NULL	NULL	0	NULL	openness 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ICNP case study demonstrated both the applicability of the TQI model and the appropriateness of the criteria identified in the TQI model : openness and responsiveness , clarity and reproducibility , understandability , accessibility and usability , interoperability , and quality of documentation .
	manualset3
153453	8	408280	13	NULL	NULL	0	NULL	responsiveness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ICNP case study demonstrated both the applicability of the TQI model and the appropriateness of the criteria identified in the TQI model : openness and responsiveness , clarity and reproducibility , understandability , accessibility and usability , interoperability , and quality of documentation .
	manualset3
153454	9	408280	13	NULL	NULL	0	NULL	 clarity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ICNP case study demonstrated both the applicability of the TQI model and the appropriateness of the criteria identified in the TQI model : openness and responsiveness , clarity and reproducibility , understandability , accessibility and usability , interoperability , and quality of documentation .
	manualset3
153455	10	408280	13	NULL	NULL	0	NULL	reproducibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ICNP case study demonstrated both the applicability of the TQI model and the appropriateness of the criteria identified in the TQI model : openness and responsiveness , clarity and reproducibility , understandability , accessibility and usability , interoperability , and quality of documentation .
	manualset3
153456	11	408280	13	NULL	NULL	0	NULL	understandability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ICNP case study demonstrated both the applicability of the TQI model and the appropriateness of the criteria identified in the TQI model : openness and responsiveness , clarity and reproducibility , understandability , accessibility and usability , interoperability , and quality of documentation .
	manualset3
153457	12	408280	13	NULL	NULL	0	NULL	 accessibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ICNP case study demonstrated both the applicability of the TQI model and the appropriateness of the criteria identified in the TQI model : openness and responsiveness , clarity and reproducibility , understandability , accessibility and usability , interoperability , and quality of documentation .
	manualset3
153458	13	408280	13	NULL	NULL	0	NULL	usability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ICNP case study demonstrated both the applicability of the TQI model and the appropriateness of the criteria identified in the TQI model : openness and responsiveness , clarity and reproducibility , understandability , accessibility and usability , interoperability , and quality of documentation .
	manualset3
153459	14	408280	13	NULL	NULL	0	NULL	interoperability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ICNP case study demonstrated both the applicability of the TQI model and the appropriateness of the criteria identified in the TQI model : openness and responsiveness , clarity and reproducibility , understandability , accessibility and usability , interoperability , and quality of documentation .
	manualset3
153460	15	408280	13	NULL	NULL	0	NULL	quality of documentation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ICNP case study demonstrated both the applicability of the TQI model and the appropriateness of the criteria identified in the TQI model : openness and responsiveness , clarity and reproducibility , understandability , accessibility and usability , interoperability , and quality of documentation .
	manualset3
153461	1	408281	13	NULL	NULL	0	NULL	 IFA results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The IFA results correlated best with those obtained with the anti-E1 specific competitive ELISA ( 85.7 % ) .
	manualset3
153462	2	408281	13	NULL	NULL	0	NULL	anti-E1 specific competitive ELISA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The IFA results correlated best with those obtained with the anti-E1 specific competitive ELISA ( 85.7 % ) .
	manualset3
153463	3	408281	13	NULL	NULL	0	NULL	85.7 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The IFA results correlated best with those obtained with the anti-E1 specific competitive ELISA ( 85.7 % ) .
	manualset3
153464	1	408282	13	NULL	NULL	0	NULL	sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The IGFBP-5 mRNA 3 ' and 5 ' UTRs were cloned and their sequences searched for adenosine-uridine rich elements ( AUREs ) , elements shown to regulate RNA stability .
	manualset3
153465	2	408282	13	NULL	NULL	0	NULL	adenosine-uridine rich elements ( AUREs )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The IGFBP-5 mRNA 3 ' and 5 ' UTRs were cloned and their sequences searched for adenosine-uridine rich elements ( AUREs ) , elements shown to regulate RNA stability .
	manualset3
153466	3	408282	13	NULL	NULL	0	NULL	elements 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The IGFBP-5 mRNA 3 ' and 5 ' UTRs were cloned and their sequences searched for adenosine-uridine rich elements ( AUREs ) , elements shown to regulate RNA stability .
	manualset3
153467	4	408282	13	NULL	NULL	0	NULL	RNA stability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The IGFBP-5 mRNA 3 ' and 5 ' UTRs were cloned and their sequences searched for adenosine-uridine rich elements ( AUREs ) , elements shown to regulate RNA stability .
	manualset3
153468	5	408282	13	NULL	NULL	0	NULL	IGFBP-5 mRNA 3 'UTRs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The IGFBP-5 mRNA 3 ' and 5 ' UTRs were cloned and their sequences searched for adenosine-uridine rich elements ( AUREs ) , elements shown to regulate RNA stability .
	manualset3
153469	6	408282	13	NULL	NULL	0	NULL	IGFBP-5 mRNA 5 ' UTRs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The IGFBP-5 mRNA 3 ' and 5 ' UTRs were cloned and their sequences searched for adenosine-uridine rich elements ( AUREs ) , elements shown to regulate RNA stability .
	manualset3
153470	1	408283	13	NULL	NULL	0	NULL	IMRT techniques 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The IMRT techniques DMLC , MIMiC and MSF were compared for the organs at risk : rectum , bladder , and left and right femoral heads .
	manualset3
153471	2	408283	13	NULL	NULL	0	NULL	DMLC	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The IMRT techniques DMLC , MIMiC and MSF were compared for the organs at risk : rectum , bladder , and left and right femoral heads .
	manualset3
153472	3	408283	13	NULL	NULL	0	NULL	MIMiC	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The IMRT techniques DMLC , MIMiC and MSF were compared for the organs at risk : rectum , bladder , and left and right femoral heads .
	manualset3
153473	4	408283	13	NULL	NULL	0	NULL	MSF 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The IMRT techniques DMLC , MIMiC and MSF were compared for the organs at risk : rectum , bladder , and left and right femoral heads .
	manualset3
153474	5	408283	13	NULL	NULL	0	NULL	organs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The IMRT techniques DMLC , MIMiC and MSF were compared for the organs at risk : rectum , bladder , and left and right femoral heads .
	manualset3
153475	6	408283	13	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The IMRT techniques DMLC , MIMiC and MSF were compared for the organs at risk : rectum , bladder , and left and right femoral heads .
	manualset3
153476	7	408283	13	NULL	NULL	0	NULL	rectum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The IMRT techniques DMLC , MIMiC and MSF were compared for the organs at risk : rectum , bladder , and left and right femoral heads .
	manualset3
153477	8	408283	13	NULL	NULL	0	NULL	bladder	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The IMRT techniques DMLC , MIMiC and MSF were compared for the organs at risk : rectum , bladder , and left and right femoral heads .
	manualset3
153478	9	408283	13	NULL	NULL	0	NULL	left femoral heads	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The IMRT techniques DMLC , MIMiC and MSF were compared for the organs at risk : rectum , bladder , and left and right femoral heads .
	manualset3
153479	10	408283	13	NULL	NULL	0	NULL	right femoral heads	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The IMRT techniques DMLC , MIMiC and MSF were compared for the organs at risk : rectum , bladder , and left and right femoral heads .
	manualset3
153480	1	408284	13	NULL	NULL	0	NULL	IRPA agency	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The IRPA agency fielded several top-down projects which encouraged a multicentre and multidisciplinary approach .
	manualset3
153481	2	408284	13	NULL	NULL	0	NULL	projects	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The IRPA agency fielded several top-down projects which encouraged a multicentre and multidisciplinary approach .
	manualset3
153482	3	408284	13	NULL	NULL	NULL	NULL	approach	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The IRPA agency fielded several top-down projects which encouraged a multicentre and multidisciplinary approach .
	manualset3
153483	1	408285	13	NULL	NULL	0	NULL	ISFI 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The ISFI was prepared by dissolving PLGA in N-methyl-2-pyrrolidone ( NMP ) or mixtures of NMP and triacetin .
	manualset3
153484	2	408285	13	NULL	NULL	0	NULL	PLGA 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ISFI was prepared by dissolving PLGA in N-methyl-2-pyrrolidone ( NMP ) or mixtures of NMP and triacetin .
	manualset3
153485	3	408285	13	NULL	NULL	0	NULL	N-methyl-2-pyrrolidone ( NMP )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ISFI was prepared by dissolving PLGA in N-methyl-2-pyrrolidone ( NMP ) or mixtures of NMP and triacetin .
	manualset3
153486	4	408285	13	NULL	NULL	0	NULL	mixtures 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ISFI was prepared by dissolving PLGA in N-methyl-2-pyrrolidone ( NMP ) or mixtures of NMP and triacetin .
	manualset3
153487	5	408285	13	NULL	NULL	0	NULL	NMP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ISFI was prepared by dissolving PLGA in N-methyl-2-pyrrolidone ( NMP ) or mixtures of NMP and triacetin .
	manualset3
153488	6	408285	13	NULL	NULL	0	NULL	triacetin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ISFI was prepared by dissolving PLGA in N-methyl-2-pyrrolidone ( NMP ) or mixtures of NMP and triacetin .
	manualset3
153489	1	408286	13	NULL	NULL	0	NULL	ISHs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The ISHs are a rare complication of head traumas .
	manualset3
153490	2	408286	13	NULL	NULL	0	NULL	complication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The ISHs are a rare complication of head traumas .
	manualset3
153491	3	408286	13	NULL	NULL	0	NULL	head traumas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The ISHs are a rare complication of head traumas .
	manualset3
153492	1	408287	13	NULL	NULL	0	NULL	 IUB ( MB )	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The IUB ( MB ) : 1955 -- 2005 .
	manualset3
153493	2	408287	13	NULL	NULL	0	NULL	1955 -- 2005	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The IUB ( MB ) : 1955 -- 2005 .
	manualset3
153494	1	408288	13	NULL	NULL	0	NULL	IkappaBa mutant 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The IkappaBa mutant was observed in cells transfected with the mutated IkappaBa gene .
	manualset3
153495	2	408288	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The IkappaBa mutant was observed in cells transfected with the mutated IkappaBa gene .
	manualset3
153496	3	408288	13	NULL	NULL	0	NULL	mutated IkappaBa gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The IkappaBa mutant was observed in cells transfected with the mutated IkappaBa gene .
	manualset3
153497	1	408289	13	NULL	NULL	0	NULL	Indonesian government 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The Indonesian government decided to reintroduce these surveys in 1977 under the name of chase or trace surveys .
	manualset3
153498	2	408289	13	NULL	NULL	0	NULL	 surveys	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Indonesian government decided to reintroduce these surveys in 1977 under the name of chase or trace surveys .
	manualset3
153499	3	408289	13	NULL	NULL	0	NULL	1977	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The Indonesian government decided to reintroduce these surveys in 1977 under the name of chase or trace surveys .
	manualset3
153500	4	408289	13	NULL	NULL	0	NULL	name	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Indonesian government decided to reintroduce these surveys in 1977 under the name of chase or trace surveys .
	manualset3
153501	5	408289	13	NULL	NULL	0	NULL	chase surveys	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Indonesian government decided to reintroduce these surveys in 1977 under the name of chase or trace surveys .
	manualset3
153502	6	408289	13	NULL	NULL	0	NULL	trace surveys	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Indonesian government decided to reintroduce these surveys in 1977 under the name of chase or trace surveys .
	manualset3
153503	1	408290	13	NULL	NULL	0	NULL	 JAK2 allele	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The JAK2 allele burdens in the patients with myeloproliferative neoplasms measured by ABC-PCR and AS-qPCR showed a good fitting .
	manualset3
153504	2	408290	13	NULL	NULL	0	NULL	burdens	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The JAK2 allele burdens in the patients with myeloproliferative neoplasms measured by ABC-PCR and AS-qPCR showed a good fitting .
	manualset3
153505	3	408290	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The JAK2 allele burdens in the patients with myeloproliferative neoplasms measured by ABC-PCR and AS-qPCR showed a good fitting .
	manualset3
153506	4	408290	13	NULL	NULL	0	NULL	myeloproliferative neoplasms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The JAK2 allele burdens in the patients with myeloproliferative neoplasms measured by ABC-PCR and AS-qPCR showed a good fitting .
	manualset3
153507	5	408290	13	NULL	NULL	0	NULL	ABC-PCR 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The JAK2 allele burdens in the patients with myeloproliferative neoplasms measured by ABC-PCR and AS-qPCR showed a good fitting .
	manualset3
153508	6	408290	13	NULL	NULL	0	NULL	AS-qPCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The JAK2 allele burdens in the patients with myeloproliferative neoplasms measured by ABC-PCR and AS-qPCR showed a good fitting .
	manualset3
153509	7	408290	13	NULL	NULL	0	NULL	good fitting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The JAK2 allele burdens in the patients with myeloproliferative neoplasms measured by ABC-PCR and AS-qPCR showed a good fitting .
	manualset3
153510	1	408291	13	NULL	NULL	0	NULL	Jak2 ( V617F ) mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Jak2 ( V617F ) mutation is found in most classical BCR/ABL-negative myeloproliferative neoplasms ( MPNs ) .
	manualset3
153511	2	408291	13	NULL	NULL	0	NULL	classical BCR/ABL-negative myeloproliferative neoplasms ( MPNs ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Jak2 ( V617F ) mutation is found in most classical BCR/ABL-negative myeloproliferative neoplasms ( MPNs ) .
	manualset3
153512	1	408292	13	NULL	NULL	0	NULL	 K130L myosin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The K130L myosin purified from these cells displays maximal actin-activated ATPase activities and promotes maximal sliding velocities of actin filaments in an in vitro motility assay that are comparable with those of wild-type myosin .
	manualset3
153513	2	408292	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The K130L myosin purified from these cells displays maximal actin-activated ATPase activities and promotes maximal sliding velocities of actin filaments in an in vitro motility assay that are comparable with those of wild-type myosin .
	manualset3
153514	3	408292	13	NULL	NULL	0	NULL	displays	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The K130L myosin purified from these cells displays maximal actin-activated ATPase activities and promotes maximal sliding velocities of actin filaments in an in vitro motility assay that are comparable with those of wild-type myosin .
	manualset3
153515	4	408292	13	NULL	NULL	0	NULL	actin-activated ATPase activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The K130L myosin purified from these cells displays maximal actin-activated ATPase activities and promotes maximal sliding velocities of actin filaments in an in vitro motility assay that are comparable with those of wild-type myosin .
	manualset3
153516	5	408292	13	NULL	NULL	0	NULL	velocities 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The K130L myosin purified from these cells displays maximal actin-activated ATPase activities and promotes maximal sliding velocities of actin filaments in an in vitro motility assay that are comparable with those of wild-type myosin .
	manualset3
153517	6	408292	13	NULL	NULL	0	NULL	actin filaments	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The K130L myosin purified from these cells displays maximal actin-activated ATPase activities and promotes maximal sliding velocities of actin filaments in an in vitro motility assay that are comparable with those of wild-type myosin .
	manualset3
153518	7	408292	13	NULL	NULL	0	NULL	in vitro motility assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The K130L myosin purified from these cells displays maximal actin-activated ATPase activities and promotes maximal sliding velocities of actin filaments in an in vitro motility assay that are comparable with those of wild-type myosin .
	manualset3
153519	8	408292	13	NULL	NULL	0	NULL	wild-type myosin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The K130L myosin purified from these cells displays maximal actin-activated ATPase activities and promotes maximal sliding velocities of actin filaments in an in vitro motility assay that are comparable with those of wild-type myosin .
	manualset3
153520	1	408293	13	NULL	NULL	0	NULL	KEGG RPAIR database	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The KEGG RPAIR database is a collection of biochemical structure transformation patterns , called RDM patterns , and chemical structure alignments of substrate-product pairs ( reactant pairs ) in all known enzyme-catalyzed reactions taken from the Enzyme Nomenclature and the KEGG PATHWAY database .
	manualset3
153521	2	408293	13	NULL	NULL	0	NULL	collection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The KEGG RPAIR database is a collection of biochemical structure transformation patterns , called RDM patterns , and chemical structure alignments of substrate-product pairs ( reactant pairs ) in all known enzyme-catalyzed reactions taken from the Enzyme Nomenclature and the KEGG PATHWAY database .
	manualset3
153522	3	408293	13	NULL	NULL	0	NULL	biochemical structure transformation patterns	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The KEGG RPAIR database is a collection of biochemical structure transformation patterns , called RDM patterns , and chemical structure alignments of substrate-product pairs ( reactant pairs ) in all known enzyme-catalyzed reactions taken from the Enzyme Nomenclature and the KEGG PATHWAY database .
	manualset3
153523	4	408293	13	NULL	NULL	0	NULL	RDM patterns	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The KEGG RPAIR database is a collection of biochemical structure transformation patterns , called RDM patterns , and chemical structure alignments of substrate-product pairs ( reactant pairs ) in all known enzyme-catalyzed reactions taken from the Enzyme Nomenclature and the KEGG PATHWAY database .
	manualset3
153524	5	408293	13	NULL	NULL	0	NULL	 chemical structure alignments 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The KEGG RPAIR database is a collection of biochemical structure transformation patterns , called RDM patterns , and chemical structure alignments of substrate-product pairs ( reactant pairs ) in all known enzyme-catalyzed reactions taken from the Enzyme Nomenclature and the KEGG PATHWAY database .
	manualset3
153525	6	408293	13	NULL	NULL	NULL	NULL	substrate-product pairs 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The KEGG RPAIR database is a collection of biochemical structure transformation patterns , called RDM patterns , and chemical structure alignments of substrate-product pairs ( reactant pairs ) in all known enzyme-catalyzed reactions taken from the Enzyme Nomenclature and the KEGG PATHWAY database .
	manualset3
153526	7	408293	13	NULL	NULL	0	NULL	reactant pairs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The KEGG RPAIR database is a collection of biochemical structure transformation patterns , called RDM patterns , and chemical structure alignments of substrate-product pairs ( reactant pairs ) in all known enzyme-catalyzed reactions taken from the Enzyme Nomenclature and the KEGG PATHWAY database .
	manualset3
153527	8	408293	13	NULL	NULL	0	NULL	enzyme-catalyzed reactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The KEGG RPAIR database is a collection of biochemical structure transformation patterns , called RDM patterns , and chemical structure alignments of substrate-product pairs ( reactant pairs ) in all known enzyme-catalyzed reactions taken from the Enzyme Nomenclature and the KEGG PATHWAY database .
	manualset3
153528	9	408293	13	NULL	NULL	0	NULL	Enzyme Nomenclature 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The KEGG RPAIR database is a collection of biochemical structure transformation patterns , called RDM patterns , and chemical structure alignments of substrate-product pairs ( reactant pairs ) in all known enzyme-catalyzed reactions taken from the Enzyme Nomenclature and the KEGG PATHWAY database .
	manualset3
153529	10	408293	13	NULL	NULL	0	NULL	KEGG PATHWAY database	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The KEGG RPAIR database is a collection of biochemical structure transformation patterns , called RDM patterns , and chemical structure alignments of substrate-product pairs ( reactant pairs ) in all known enzyme-catalyzed reactions taken from the Enzyme Nomenclature and the KEGG PATHWAY database .
	manualset3
153530	1	408294	13	NULL	NULL	0	NULL	Kd values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Kd and Bmax values in the subregions of the gerbil hippocampus were estimated at 2.6-3 .8 nM and 2.38-2 .54 pmol ( mg tissue ) -1 , respectively .
	manualset3
153531	2	408294	13	NULL	NULL	0	NULL	Bmax values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Kd and Bmax values in the subregions of the gerbil hippocampus were estimated at 2.6-3 .8 nM and 2.38-2 .54 pmol ( mg tissue ) -1 , respectively .
	manualset3
153532	3	408294	13	NULL	NULL	0	NULL	subregions 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The Kd and Bmax values in the subregions of the gerbil hippocampus were estimated at 2.6-3 .8 nM and 2.38-2 .54 pmol ( mg tissue ) -1 , respectively .
	manualset3
153533	4	408294	13	NULL	NULL	0	NULL	gerbil hippocampus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The Kd and Bmax values in the subregions of the gerbil hippocampus were estimated at 2.6-3 .8 nM and 2.38-2 .54 pmol ( mg tissue ) -1 , respectively .
	manualset3
153534	5	408294	13	NULL	NULL	0	NULL	2.6-3 .8 nM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Kd and Bmax values in the subregions of the gerbil hippocampus were estimated at 2.6-3 .8 nM and 2.38-2 .54 pmol ( mg tissue ) -1 , respectively .
	manualset3
153535	6	408294	13	NULL	NULL	0	NULL	2.38-2 .54 pmol ( mg tissue ) -1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Kd and Bmax values in the subregions of the gerbil hippocampus were estimated at 2.6-3 .8 nM and 2.38-2 .54 pmol ( mg tissue ) -1 , respectively .
	manualset3
153536	1	408295	13	NULL	NULL	0	NULL	Kd	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Kd for ouabain binding to Na ( + ) - K ( + ) - ATPase was 7.8 nM .
	manualset3
153537	2	408295	13	NULL	NULL	0	NULL	ouabain binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Kd for ouabain binding to Na ( + ) - K ( + ) - ATPase was 7.8 nM .
	manualset3
153538	3	408295	13	NULL	NULL	0	NULL	Na ( + ) - K ( + ) - ATPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The Kd for ouabain binding to Na ( + ) - K ( + ) - ATPase was 7.8 nM .
	manualset3
153539	4	408295	13	NULL	NULL	0	NULL	7.8 nM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Kd for ouabain binding to Na ( + ) - K ( + ) - ATPase was 7.8 nM .
	manualset3
153540	1	408296	13	NULL	NULL	0	NULL	Km 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Km of intracellular CO2 + uptake was lower in the case of adapted cells as compared with the parent , whereas Vmax showed an opposite trend .
	manualset3
153541	2	408296	13	NULL	NULL	0	NULL	intracellular CO2 + uptake	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Km of intracellular CO2 + uptake was lower in the case of adapted cells as compared with the parent , whereas Vmax showed an opposite trend .
	manualset3
153542	3	408296	13	NULL	NULL	0	NULL	 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The Km of intracellular CO2 + uptake was lower in the case of adapted cells as compared with the parent , whereas Vmax showed an opposite trend .
	manualset3
153543	4	408296	13	NULL	NULL	0	NULL	parent	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The Km of intracellular CO2 + uptake was lower in the case of adapted cells as compared with the parent , whereas Vmax showed an opposite trend .
	manualset3
153544	5	408296	13	NULL	NULL	0	NULL	Vmax	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Km of intracellular CO2 + uptake was lower in the case of adapted cells as compared with the parent , whereas Vmax showed an opposite trend .
	manualset3
153545	6	408296	13	NULL	NULL	0	NULL	opposite trend	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Km of intracellular CO2 + uptake was lower in the case of adapted cells as compared with the parent , whereas Vmax showed an opposite trend .
	manualset3
153546	1	408297	13	NULL	NULL	0	NULL	Kt 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Kt for Phe-Pro-Ala transport ( 36 + / - 3 microM ) was equal to the Ki for Phe-Pro-Ala to inhibit Gly-Sar transport ( 36 + / - 6 microM ) .
	manualset3
153547	2	408297	13	NULL	NULL	0	NULL	Phe-Pro-Ala transport	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Kt for Phe-Pro-Ala transport ( 36 + / - 3 microM ) was equal to the Ki for Phe-Pro-Ala to inhibit Gly-Sar transport ( 36 + / - 6 microM ) .
	manualset3
153548	3	408297	13	NULL	NULL	0	NULL	36 + / - 3 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Kt for Phe-Pro-Ala transport ( 36 + / - 3 microM ) was equal to the Ki for Phe-Pro-Ala to inhibit Gly-Sar transport ( 36 + / - 6 microM ) .
	manualset3
153549	4	408297	13	NULL	NULL	0	NULL	Ki 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Kt for Phe-Pro-Ala transport ( 36 + / - 3 microM ) was equal to the Ki for Phe-Pro-Ala to inhibit Gly-Sar transport ( 36 + / - 6 microM ) .
	manualset3
153550	5	408297	13	NULL	NULL	0	NULL	Phe-Pro-Ala 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The Kt for Phe-Pro-Ala transport ( 36 + / - 3 microM ) was equal to the Ki for Phe-Pro-Ala to inhibit Gly-Sar transport ( 36 + / - 6 microM ) .
	manualset3
153551	6	408297	13	NULL	NULL	0	NULL	Gly-Sar transport	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Kt for Phe-Pro-Ala transport ( 36 + / - 3 microM ) was equal to the Ki for Phe-Pro-Ala to inhibit Gly-Sar transport ( 36 + / - 6 microM ) .
	manualset3
153552	7	408297	13	NULL	NULL	0	NULL	36 + / - 6 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Kt for Phe-Pro-Ala transport ( 36 + / - 3 microM ) was equal to the Ki for Phe-Pro-Ala to inhibit Gly-Sar transport ( 36 + / - 6 microM ) .
	manualset3
153553	1	408298	13	NULL	NULL	0	NULL	L1 ORF	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The L1 ORF of HPV18 genomes had an increased proportion of nonsynonymous substitutions ( 4.93 % ; average d ( N ) / d ( S ) ratio ( M3 ) = 0.3356 ) compared to HPV45 ( 1.86 % ; M3 = 0.1268 ) and HPV16 ( 2.26 % ; M3 = 0.1330 ) L1 ORFs .
	manualset3
153554	2	408298	13	NULL	NULL	0	NULL	HPV18 genomes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The L1 ORF of HPV18 genomes had an increased proportion of nonsynonymous substitutions ( 4.93 % ; average d ( N ) / d ( S ) ratio ( M3 ) = 0.3356 ) compared to HPV45 ( 1.86 % ; M3 = 0.1268 ) and HPV16 ( 2.26 % ; M3 = 0.1330 ) L1 ORFs .
	manualset3
153555	3	408298	13	NULL	NULL	0	NULL	proportion	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The L1 ORF of HPV18 genomes had an increased proportion of nonsynonymous substitutions ( 4.93 % ; average d ( N ) / d ( S ) ratio ( M3 ) = 0.3356 ) compared to HPV45 ( 1.86 % ; M3 = 0.1268 ) and HPV16 ( 2.26 % ; M3 = 0.1330 ) L1 ORFs .
	manualset3
153556	4	408298	13	NULL	NULL	0	NULL	nonsynonymous substitutions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The L1 ORF of HPV18 genomes had an increased proportion of nonsynonymous substitutions ( 4.93 % ; average d ( N ) / d ( S ) ratio ( M3 ) = 0.3356 ) compared to HPV45 ( 1.86 % ; M3 = 0.1268 ) and HPV16 ( 2.26 % ; M3 = 0.1330 ) L1 ORFs .
	manualset3
153557	5	408298	13	NULL	NULL	0	NULL	4.93 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The L1 ORF of HPV18 genomes had an increased proportion of nonsynonymous substitutions ( 4.93 % ; average d ( N ) / d ( S ) ratio ( M3 ) = 0.3356 ) compared to HPV45 ( 1.86 % ; M3 = 0.1268 ) and HPV16 ( 2.26 % ; M3 = 0.1330 ) L1 ORFs .
	manualset3
153558	6	408298	13	NULL	NULL	0	NULL	 average d ( N ) / d ( S ) ratio ( M3 ) = 0.3356	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The L1 ORF of HPV18 genomes had an increased proportion of nonsynonymous substitutions ( 4.93 % ; average d ( N ) / d ( S ) ratio ( M3 ) = 0.3356 ) compared to HPV45 ( 1.86 % ; M3 = 0.1268 ) and HPV16 ( 2.26 % ; M3 = 0.1330 ) L1 ORFs .
	manualset3
153559	7	408298	13	NULL	NULL	0	NULL	HPV45 L1 ORFs 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The L1 ORF of HPV18 genomes had an increased proportion of nonsynonymous substitutions ( 4.93 % ; average d ( N ) / d ( S ) ratio ( M3 ) = 0.3356 ) compared to HPV45 ( 1.86 % ; M3 = 0.1268 ) and HPV16 ( 2.26 % ; M3 = 0.1330 ) L1 ORFs .
	manualset3
153560	8	408298	13	NULL	NULL	0	NULL	1.86 % ; M3 = 0.1268 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The L1 ORF of HPV18 genomes had an increased proportion of nonsynonymous substitutions ( 4.93 % ; average d ( N ) / d ( S ) ratio ( M3 ) = 0.3356 ) compared to HPV45 ( 1.86 % ; M3 = 0.1268 ) and HPV16 ( 2.26 % ; M3 = 0.1330 ) L1 ORFs .
	manualset3
153561	9	408298	13	NULL	NULL	0	NULL	HPV16 L1 ORFs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The L1 ORF of HPV18 genomes had an increased proportion of nonsynonymous substitutions ( 4.93 % ; average d ( N ) / d ( S ) ratio ( M3 ) = 0.3356 ) compared to HPV45 ( 1.86 % ; M3 = 0.1268 ) and HPV16 ( 2.26 % ; M3 = 0.1330 ) L1 ORFs .
	manualset3
153562	10	408298	13	NULL	NULL	0	NULL	2.26 % ; M3 = 0.1330	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The L1 ORF of HPV18 genomes had an increased proportion of nonsynonymous substitutions ( 4.93 % ; average d ( N ) / d ( S ) ratio ( M3 ) = 0.3356 ) compared to HPV45 ( 1.86 % ; M3 = 0.1268 ) and HPV16 ( 2.26 % ; M3 = 0.1330 ) L1 ORFs .
	manualset3
153563	1	408299	13	NULL	NULL	0	NULL	LAL-test	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The LAL-test is considered to constitute a valuable cow-side test for the veterinary practitioner , aiding the selection of antibacterial drug of choice for the initial treatment of clinical mastitis .
	manualset3
153564	2	408299	13	NULL	NULL	0	NULL	cow-side test 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The LAL-test is considered to constitute a valuable cow-side test for the veterinary practitioner , aiding the selection of antibacterial drug of choice for the initial treatment of clinical mastitis .
	manualset3
153565	3	408299	13	NULL	NULL	0	NULL	veterinary practitioner	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The LAL-test is considered to constitute a valuable cow-side test for the veterinary practitioner , aiding the selection of antibacterial drug of choice for the initial treatment of clinical mastitis .
	manualset3
153566	4	408299	13	NULL	NULL	0	NULL	 selection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The LAL-test is considered to constitute a valuable cow-side test for the veterinary practitioner , aiding the selection of antibacterial drug of choice for the initial treatment of clinical mastitis .
	manualset3
153567	5	408299	13	NULL	NULL	0	NULL	antibacterial drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The LAL-test is considered to constitute a valuable cow-side test for the veterinary practitioner , aiding the selection of antibacterial drug of choice for the initial treatment of clinical mastitis .
	manualset3
153568	6	408299	13	NULL	NULL	0	NULL	choice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The LAL-test is considered to constitute a valuable cow-side test for the veterinary practitioner , aiding the selection of antibacterial drug of choice for the initial treatment of clinical mastitis .
	manualset3
153569	7	408299	13	NULL	NULL	0	NULL	initial treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The LAL-test is considered to constitute a valuable cow-side test for the veterinary practitioner , aiding the selection of antibacterial drug of choice for the initial treatment of clinical mastitis .
	manualset3
153570	8	408299	13	NULL	NULL	0	NULL	clinical mastitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The LAL-test is considered to constitute a valuable cow-side test for the veterinary practitioner , aiding the selection of antibacterial drug of choice for the initial treatment of clinical mastitis .
	manualset3
153571	1	408300	13	NULL	NULL	0	NULL	LAM-1 + memory cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The LAM-1 + memory cells proliferated better to recall antigen and induced three to seven times higher levels of B cell immunoglobulin secretion than their LAM-1 - counterparts .
	manualset3
153572	2	408300	13	NULL	NULL	0	NULL	antigen 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The LAM-1 + memory cells proliferated better to recall antigen and induced three to seven times higher levels of B cell immunoglobulin secretion than their LAM-1 - counterparts .
	manualset3
153573	3	408300	13	NULL	NULL	0	NULL	three to seven times 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The LAM-1 + memory cells proliferated better to recall antigen and induced three to seven times higher levels of B cell immunoglobulin secretion than their LAM-1 - counterparts .
	manualset3
153574	4	408300	13	NULL	NULL	0	NULL	 levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The LAM-1 + memory cells proliferated better to recall antigen and induced three to seven times higher levels of B cell immunoglobulin secretion than their LAM-1 - counterparts .
	manualset3
153575	5	408300	13	NULL	NULL	0	NULL	B cell immunoglobulin secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The LAM-1 + memory cells proliferated better to recall antigen and induced three to seven times higher levels of B cell immunoglobulin secretion than their LAM-1 - counterparts .
	manualset3
153576	6	408300	13	NULL	NULL	0	NULL	LAM-1 - counterparts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The LAM-1 + memory cells proliferated better to recall antigen and induced three to seven times higher levels of B cell immunoglobulin secretion than their LAM-1 - counterparts .
	manualset3
153577	1	408301	13	NULL	NULL	0	NULL	 LAT	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The LAT evaluated here was no more specific than the double-immunodiffusion assay .
	manualset3
153578	2	408301	13	NULL	NULL	0	NULL	double-immunodiffusion assay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The LAT evaluated here was no more specific than the double-immunodiffusion assay .
	manualset3
153579	1	408302	13	NULL	NULL	0	NULL	LC ( 50 ) values 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The LC ( 50 ) values ranged from 1757 microg l ( -1 ) for naphthalene after 10 d exposure to 79.1 microg l ( -1 ) for pyrene after 28 d exposure , and the EC ( 50 ) ranged from 1587 microg l ( -1 ) for naphthalene after 10 d exposure to 38.2 microg l ( -1 ) for pyrene after 28 d exposure .
	manualset3
153580	2	408302	13	NULL	NULL	0	NULL	1757 microg l ( -1 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The LC ( 50 ) values ranged from 1757 microg l ( -1 ) for naphthalene after 10 d exposure to 79.1 microg l ( -1 ) for pyrene after 28 d exposure , and the EC ( 50 ) ranged from 1587 microg l ( -1 ) for naphthalene after 10 d exposure to 38.2 microg l ( -1 ) for pyrene after 28 d exposure .
	manualset3
153581	3	408302	13	NULL	NULL	0	NULL	naphthalene 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The LC ( 50 ) values ranged from 1757 microg l ( -1 ) for naphthalene after 10 d exposure to 79.1 microg l ( -1 ) for pyrene after 28 d exposure , and the EC ( 50 ) ranged from 1587 microg l ( -1 ) for naphthalene after 10 d exposure to 38.2 microg l ( -1 ) for pyrene after 28 d exposure .
	manualset3
153582	4	408302	13	NULL	NULL	0	NULL	10 d 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The LC ( 50 ) values ranged from 1757 microg l ( -1 ) for naphthalene after 10 d exposure to 79.1 microg l ( -1 ) for pyrene after 28 d exposure , and the EC ( 50 ) ranged from 1587 microg l ( -1 ) for naphthalene after 10 d exposure to 38.2 microg l ( -1 ) for pyrene after 28 d exposure .
	manualset3
153583	5	408302	13	NULL	NULL	0	NULL	exposure 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The LC ( 50 ) values ranged from 1757 microg l ( -1 ) for naphthalene after 10 d exposure to 79.1 microg l ( -1 ) for pyrene after 28 d exposure , and the EC ( 50 ) ranged from 1587 microg l ( -1 ) for naphthalene after 10 d exposure to 38.2 microg l ( -1 ) for pyrene after 28 d exposure .
	manualset3
153584	6	408302	13	NULL	NULL	0	NULL	79.1 microg l ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The LC ( 50 ) values ranged from 1757 microg l ( -1 ) for naphthalene after 10 d exposure to 79.1 microg l ( -1 ) for pyrene after 28 d exposure , and the EC ( 50 ) ranged from 1587 microg l ( -1 ) for naphthalene after 10 d exposure to 38.2 microg l ( -1 ) for pyrene after 28 d exposure .
	manualset3
153585	7	408302	13	NULL	NULL	0	NULL	pyrene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The LC ( 50 ) values ranged from 1757 microg l ( -1 ) for naphthalene after 10 d exposure to 79.1 microg l ( -1 ) for pyrene after 28 d exposure , and the EC ( 50 ) ranged from 1587 microg l ( -1 ) for naphthalene after 10 d exposure to 38.2 microg l ( -1 ) for pyrene after 28 d exposure .
	manualset3
153586	8	408302	13	NULL	NULL	0	NULL	28 d 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The LC ( 50 ) values ranged from 1757 microg l ( -1 ) for naphthalene after 10 d exposure to 79.1 microg l ( -1 ) for pyrene after 28 d exposure , and the EC ( 50 ) ranged from 1587 microg l ( -1 ) for naphthalene after 10 d exposure to 38.2 microg l ( -1 ) for pyrene after 28 d exposure .
	manualset3
153587	9	408302	13	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The LC ( 50 ) values ranged from 1757 microg l ( -1 ) for naphthalene after 10 d exposure to 79.1 microg l ( -1 ) for pyrene after 28 d exposure , and the EC ( 50 ) ranged from 1587 microg l ( -1 ) for naphthalene after 10 d exposure to 38.2 microg l ( -1 ) for pyrene after 28 d exposure .
	manualset3
153588	10	408302	13	NULL	NULL	0	NULL	EC ( 50 ) 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The LC ( 50 ) values ranged from 1757 microg l ( -1 ) for naphthalene after 10 d exposure to 79.1 microg l ( -1 ) for pyrene after 28 d exposure , and the EC ( 50 ) ranged from 1587 microg l ( -1 ) for naphthalene after 10 d exposure to 38.2 microg l ( -1 ) for pyrene after 28 d exposure .
	manualset3
153589	11	408302	13	NULL	NULL	0	NULL	1587 microg l ( -1 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The LC ( 50 ) values ranged from 1757 microg l ( -1 ) for naphthalene after 10 d exposure to 79.1 microg l ( -1 ) for pyrene after 28 d exposure , and the EC ( 50 ) ranged from 1587 microg l ( -1 ) for naphthalene after 10 d exposure to 38.2 microg l ( -1 ) for pyrene after 28 d exposure .
	manualset3
153590	12	408302	13	NULL	NULL	0	NULL	naphthalene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The LC ( 50 ) values ranged from 1757 microg l ( -1 ) for naphthalene after 10 d exposure to 79.1 microg l ( -1 ) for pyrene after 28 d exposure , and the EC ( 50 ) ranged from 1587 microg l ( -1 ) for naphthalene after 10 d exposure to 38.2 microg l ( -1 ) for pyrene after 28 d exposure .
	manualset3
153591	13	408302	13	NULL	NULL	0	NULL	10 d	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The LC ( 50 ) values ranged from 1757 microg l ( -1 ) for naphthalene after 10 d exposure to 79.1 microg l ( -1 ) for pyrene after 28 d exposure , and the EC ( 50 ) ranged from 1587 microg l ( -1 ) for naphthalene after 10 d exposure to 38.2 microg l ( -1 ) for pyrene after 28 d exposure .
	manualset3
153592	14	408302	13	NULL	NULL	0	NULL	exposure 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The LC ( 50 ) values ranged from 1757 microg l ( -1 ) for naphthalene after 10 d exposure to 79.1 microg l ( -1 ) for pyrene after 28 d exposure , and the EC ( 50 ) ranged from 1587 microg l ( -1 ) for naphthalene after 10 d exposure to 38.2 microg l ( -1 ) for pyrene after 28 d exposure .
	manualset3
153593	15	408302	13	NULL	NULL	0	NULL	38.2 microg l ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The LC ( 50 ) values ranged from 1757 microg l ( -1 ) for naphthalene after 10 d exposure to 79.1 microg l ( -1 ) for pyrene after 28 d exposure , and the EC ( 50 ) ranged from 1587 microg l ( -1 ) for naphthalene after 10 d exposure to 38.2 microg l ( -1 ) for pyrene after 28 d exposure .
	manualset3
153594	16	408302	13	NULL	NULL	0	NULL	pyrene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The LC ( 50 ) values ranged from 1757 microg l ( -1 ) for naphthalene after 10 d exposure to 79.1 microg l ( -1 ) for pyrene after 28 d exposure , and the EC ( 50 ) ranged from 1587 microg l ( -1 ) for naphthalene after 10 d exposure to 38.2 microg l ( -1 ) for pyrene after 28 d exposure .
	manualset3
153595	17	408302	13	NULL	NULL	0	NULL	28 d 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The LC ( 50 ) values ranged from 1757 microg l ( -1 ) for naphthalene after 10 d exposure to 79.1 microg l ( -1 ) for pyrene after 28 d exposure , and the EC ( 50 ) ranged from 1587 microg l ( -1 ) for naphthalene after 10 d exposure to 38.2 microg l ( -1 ) for pyrene after 28 d exposure .
	manualset3
153596	18	408302	13	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The LC ( 50 ) values ranged from 1757 microg l ( -1 ) for naphthalene after 10 d exposure to 79.1 microg l ( -1 ) for pyrene after 28 d exposure , and the EC ( 50 ) ranged from 1587 microg l ( -1 ) for naphthalene after 10 d exposure to 38.2 microg l ( -1 ) for pyrene after 28 d exposure .
	manualset3
153597	1	408303	13	NULL	NULL	0	NULL	LC50 estimates	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The LC50 estimates were in the range of 0.0020-0 .0067 microg ( AI ) / ml .
	manualset3
153598	2	408303	13	NULL	NULL	0	NULL	range of 0.0020-0 .0067 microg ( AI ) / ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The LC50 estimates were in the range of 0.0020-0 .0067 microg ( AI ) / ml .
	manualset3
153599	1	408304	13	NULL	NULL	0	NULL	receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A receptor for cachectin was identified on non-tumorigenic cultured cells and on normal mouse liver membranes .
	manualset3
153600	2	408304	13	NULL	NULL	0	NULL	cachectin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A receptor for cachectin was identified on non-tumorigenic cultured cells and on normal mouse liver membranes .
	manualset3
153601	3	408304	13	NULL	NULL	0	NULL	non-tumorigenic cultured cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A receptor for cachectin was identified on non-tumorigenic cultured cells and on normal mouse liver membranes .
	manualset3
153602	4	408304	13	NULL	NULL	0	NULL	normal mouse liver membranes 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A receptor for cachectin was identified on non-tumorigenic cultured cells and on normal mouse liver membranes .
	manualset3
153603	1	408305	13	NULL	NULL	0	NULL	LD 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The LD of 24-month old foals had lower phospholipids content ( p0 .001 ) , displayed little difference in saturated fatty acids ( SFA ) ( p0 .1 ) , exhibited higher levels of monounsaturated fatty acids ( MUFA ) ( p0 .05 ) and lower levels of polyunsaturated fatty acids ( PUFA ) ( p0 .05 ) compared with that of the 16-month old foals .
	manualset3
153604	2	408305	13	NULL	NULL	0	NULL	24-month old foals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The LD of 24-month old foals had lower phospholipids content ( p0 .001 ) , displayed little difference in saturated fatty acids ( SFA ) ( p0 .1 ) , exhibited higher levels of monounsaturated fatty acids ( MUFA ) ( p0 .05 ) and lower levels of polyunsaturated fatty acids ( PUFA ) ( p0 .05 ) compared with that of the 16-month old foals .
	manualset3
153605	3	408305	13	NULL	NULL	0	NULL	phospholipids content	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The LD of 24-month old foals had lower phospholipids content ( p0 .001 ) , displayed little difference in saturated fatty acids ( SFA ) ( p0 .1 ) , exhibited higher levels of monounsaturated fatty acids ( MUFA ) ( p0 .05 ) and lower levels of polyunsaturated fatty acids ( PUFA ) ( p0 .05 ) compared with that of the 16-month old foals .
	manualset3
153606	4	408305	13	NULL	NULL	0	NULL	p0 .001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The LD of 24-month old foals had lower phospholipids content ( p0 .001 ) , displayed little difference in saturated fatty acids ( SFA ) ( p0 .1 ) , exhibited higher levels of monounsaturated fatty acids ( MUFA ) ( p0 .05 ) and lower levels of polyunsaturated fatty acids ( PUFA ) ( p0 .05 ) compared with that of the 16-month old foals .
	manualset3
153607	5	408305	13	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The LD of 24-month old foals had lower phospholipids content ( p0 .001 ) , displayed little difference in saturated fatty acids ( SFA ) ( p0 .1 ) , exhibited higher levels of monounsaturated fatty acids ( MUFA ) ( p0 .05 ) and lower levels of polyunsaturated fatty acids ( PUFA ) ( p0 .05 ) compared with that of the 16-month old foals .
	manualset3
153608	6	408305	13	NULL	NULL	0	NULL	saturated fatty acids ( SFA )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The LD of 24-month old foals had lower phospholipids content ( p0 .001 ) , displayed little difference in saturated fatty acids ( SFA ) ( p0 .1 ) , exhibited higher levels of monounsaturated fatty acids ( MUFA ) ( p0 .05 ) and lower levels of polyunsaturated fatty acids ( PUFA ) ( p0 .05 ) compared with that of the 16-month old foals .
	manualset3
153609	7	408305	13	NULL	NULL	0	NULL	p0 .1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The LD of 24-month old foals had lower phospholipids content ( p0 .001 ) , displayed little difference in saturated fatty acids ( SFA ) ( p0 .1 ) , exhibited higher levels of monounsaturated fatty acids ( MUFA ) ( p0 .05 ) and lower levels of polyunsaturated fatty acids ( PUFA ) ( p0 .05 ) compared with that of the 16-month old foals .
	manualset3
153610	8	408305	13	NULL	NULL	0	NULL	levels of monounsaturated fatty acids ( MUFA ) 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The LD of 24-month old foals had lower phospholipids content ( p0 .001 ) , displayed little difference in saturated fatty acids ( SFA ) ( p0 .1 ) , exhibited higher levels of monounsaturated fatty acids ( MUFA ) ( p0 .05 ) and lower levels of polyunsaturated fatty acids ( PUFA ) ( p0 .05 ) compared with that of the 16-month old foals .
	manualset3
153611	9	408305	13	NULL	NULL	0	NULL	p0 .05 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The LD of 24-month old foals had lower phospholipids content ( p0 .001 ) , displayed little difference in saturated fatty acids ( SFA ) ( p0 .1 ) , exhibited higher levels of monounsaturated fatty acids ( MUFA ) ( p0 .05 ) and lower levels of polyunsaturated fatty acids ( PUFA ) ( p0 .05 ) compared with that of the 16-month old foals .
	manualset3
153612	10	408305	13	NULL	NULL	0	NULL	levels of polyunsaturated fatty acids ( PUFA )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The LD of 24-month old foals had lower phospholipids content ( p0 .001 ) , displayed little difference in saturated fatty acids ( SFA ) ( p0 .1 ) , exhibited higher levels of monounsaturated fatty acids ( MUFA ) ( p0 .05 ) and lower levels of polyunsaturated fatty acids ( PUFA ) ( p0 .05 ) compared with that of the 16-month old foals .
	manualset3
153613	11	408305	13	NULL	NULL	0	NULL	p0 .05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The LD of 24-month old foals had lower phospholipids content ( p0 .001 ) , displayed little difference in saturated fatty acids ( SFA ) ( p0 .1 ) , exhibited higher levels of monounsaturated fatty acids ( MUFA ) ( p0 .05 ) and lower levels of polyunsaturated fatty acids ( PUFA ) ( p0 .05 ) compared with that of the 16-month old foals .
	manualset3
153614	12	408305	13	NULL	NULL	0	NULL	16-month old foals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The LD of 24-month old foals had lower phospholipids content ( p0 .001 ) , displayed little difference in saturated fatty acids ( SFA ) ( p0 .1 ) , exhibited higher levels of monounsaturated fatty acids ( MUFA ) ( p0 .05 ) and lower levels of polyunsaturated fatty acids ( PUFA ) ( p0 .05 ) compared with that of the 16-month old foals .
	manualset3
153615	1	408306	13	NULL	NULL	0	NULL	LDH-1 abnormality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The LDH-1 abnormality helps to meet the need for an index of cardiac rejection during the early weeks after operation when the electro-cardiogram is least reliable .
	manualset3
153616	2	408306	13	NULL	NULL	0	NULL	need 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The LDH-1 abnormality helps to meet the need for an index of cardiac rejection during the early weeks after operation when the electro-cardiogram is least reliable .
	manualset3
153617	3	408306	13	NULL	NULL	0	NULL	index 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The LDH-1 abnormality helps to meet the need for an index of cardiac rejection during the early weeks after operation when the electro-cardiogram is least reliable .
	manualset3
153618	4	408306	13	NULL	NULL	0	NULL	cardiac rejection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The LDH-1 abnormality helps to meet the need for an index of cardiac rejection during the early weeks after operation when the electro-cardiogram is least reliable .
	manualset3
153619	5	408306	13	NULL	NULL	0	NULL	early weeks 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The LDH-1 abnormality helps to meet the need for an index of cardiac rejection during the early weeks after operation when the electro-cardiogram is least reliable .
	manualset3
153620	6	408306	13	NULL	NULL	0	NULL	operation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The LDH-1 abnormality helps to meet the need for an index of cardiac rejection during the early weeks after operation when the electro-cardiogram is least reliable .
	manualset3
153621	7	408306	13	NULL	NULL	0	NULL	electro-cardiogram	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The LDH-1 abnormality helps to meet the need for an index of cardiac rejection during the early weeks after operation when the electro-cardiogram is least reliable .
	manualset3
153622	1	408307	13	NULL	NULL	0	NULL	LPD group 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The LPD group also showed gradual recovery of regional myocardial function and a decrease in the frequency of premature ventricular contractions .
	manualset3
153623	2	408307	13	NULL	NULL	0	NULL	gradual recovery 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The LPD group also showed gradual recovery of regional myocardial function and a decrease in the frequency of premature ventricular contractions .
	manualset3
153624	3	408307	13	NULL	NULL	0	NULL	regional myocardial function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The LPD group also showed gradual recovery of regional myocardial function and a decrease in the frequency of premature ventricular contractions .
	manualset3
153625	4	408307	13	NULL	NULL	0	NULL	decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The LPD group also showed gradual recovery of regional myocardial function and a decrease in the frequency of premature ventricular contractions .
	manualset3
153626	5	408307	13	NULL	NULL	0	NULL	frequency	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The LPD group also showed gradual recovery of regional myocardial function and a decrease in the frequency of premature ventricular contractions .
	manualset3
153627	6	408307	13	NULL	NULL	0	NULL	premature ventricular contractions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The LPD group also showed gradual recovery of regional myocardial function and a decrease in the frequency of premature ventricular contractions .
	manualset3
153628	1	408308	13	NULL	NULL	0	NULL	LR test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The LR test always achieved the most significant P-values , followed by the exact test .
	manualset3
153629	2	408308	13	NULL	NULL	0	NULL	P-values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The LR test always achieved the most significant P-values , followed by the exact test .
	manualset3
153630	3	408308	13	NULL	NULL	0	NULL	exact test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The LR test always achieved the most significant P-values , followed by the exact test .
	manualset3
153631	1	408309	13	NULL	NULL	0	NULL	LR	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The LR was due mainly to the T lymphocytes of the L3T4 + , Ly-2 - helper phenotype .
	manualset3
153632	2	408309	13	NULL	NULL	0	NULL	T lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The LR was due mainly to the T lymphocytes of the L3T4 + , Ly-2 - helper phenotype .
	manualset3
153633	3	408309	13	NULL	NULL	0	NULL	L3T4 + phenotype	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The LR was due mainly to the T lymphocytes of the L3T4 + , Ly-2 - helper phenotype .
	manualset3
153634	4	408309	13	NULL	NULL	0	NULL	Ly-2 - helper phenotype	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The LR was due mainly to the T lymphocytes of the L3T4 + , Ly-2 - helper phenotype .
	manualset3
153635	1	408310	13	NULL	NULL	0	NULL	LR	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The LR was not altered by terfenadine but was very significantly attenuated by salbutamol ; the mean maximum fall in FEV1 during LR being 31 , 29 and 12 % after placebo , terfenadine and salbutamol , respectively .
	manualset3
153636	2	408310	13	NULL	NULL	0	NULL	terfenadine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The LR was not altered by terfenadine but was very significantly attenuated by salbutamol ; the mean maximum fall in FEV1 during LR being 31 , 29 and 12 % after placebo , terfenadine and salbutamol , respectively .
	manualset3
153637	3	408310	13	NULL	NULL	0	NULL	salbutamol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The LR was not altered by terfenadine but was very significantly attenuated by salbutamol ; the mean maximum fall in FEV1 during LR being 31 , 29 and 12 % after placebo , terfenadine and salbutamol , respectively .
	manualset3
153638	4	408310	13	NULL	NULL	0	NULL	mean maximum fall 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The LR was not altered by terfenadine but was very significantly attenuated by salbutamol ; the mean maximum fall in FEV1 during LR being 31 , 29 and 12 % after placebo , terfenadine and salbutamol , respectively .
	manualset3
153639	5	408310	13	NULL	NULL	0	NULL	FEV1	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The LR was not altered by terfenadine but was very significantly attenuated by salbutamol ; the mean maximum fall in FEV1 during LR being 31 , 29 and 12 % after placebo , terfenadine and salbutamol , respectively .
	manualset3
153640	6	408310	13	NULL	NULL	0	NULL	LR	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The LR was not altered by terfenadine but was very significantly attenuated by salbutamol ; the mean maximum fall in FEV1 during LR being 31 , 29 and 12 % after placebo , terfenadine and salbutamol , respectively .
	manualset3
153641	7	408310	13	NULL	NULL	0	NULL	31 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The LR was not altered by terfenadine but was very significantly attenuated by salbutamol ; the mean maximum fall in FEV1 during LR being 31 , 29 and 12 % after placebo , terfenadine and salbutamol , respectively .
	manualset3
153642	8	408310	13	NULL	NULL	0	NULL	29 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The LR was not altered by terfenadine but was very significantly attenuated by salbutamol ; the mean maximum fall in FEV1 during LR being 31 , 29 and 12 % after placebo , terfenadine and salbutamol , respectively .
	manualset3
153643	9	408310	13	NULL	NULL	0	NULL	12 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The LR was not altered by terfenadine but was very significantly attenuated by salbutamol ; the mean maximum fall in FEV1 during LR being 31 , 29 and 12 % after placebo , terfenadine and salbutamol , respectively .
	manualset3
153644	10	408310	13	NULL	NULL	0	NULL	placebo	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The LR was not altered by terfenadine but was very significantly attenuated by salbutamol ; the mean maximum fall in FEV1 during LR being 31 , 29 and 12 % after placebo , terfenadine and salbutamol , respectively .
	manualset3
153645	11	408310	13	NULL	NULL	0	NULL	terfenadine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The LR was not altered by terfenadine but was very significantly attenuated by salbutamol ; the mean maximum fall in FEV1 during LR being 31 , 29 and 12 % after placebo , terfenadine and salbutamol , respectively .
	manualset3
153646	12	408310	13	NULL	NULL	0	NULL	salbutamol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The LR was not altered by terfenadine but was very significantly attenuated by salbutamol ; the mean maximum fall in FEV1 during LR being 31 , 29 and 12 % after placebo , terfenadine and salbutamol , respectively .
	manualset3
153647	1	408311	13	NULL	NULL	0	NULL	Langmuir isotherm	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Langmuir isotherm was used to describe the experimental adsorption , the maximum Cu2 + adsorption capacity of the kaolin/CA reached up to 53.63 mg/g .
	manualset3
153648	2	408311	13	NULL	NULL	0	NULL	experimental adsorption	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Langmuir isotherm was used to describe the experimental adsorption , the maximum Cu2 + adsorption capacity of the kaolin/CA reached up to 53.63 mg/g .
	manualset3
153649	3	408311	13	NULL	NULL	0	NULL	Cu2 + adsorption capacity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Langmuir isotherm was used to describe the experimental adsorption , the maximum Cu2 + adsorption capacity of the kaolin/CA reached up to 53.63 mg/g .
	manualset3
153650	4	408311	13	NULL	NULL	0	NULL	kaolin/CA 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Langmuir isotherm was used to describe the experimental adsorption , the maximum Cu2 + adsorption capacity of the kaolin/CA reached up to 53.63 mg/g .
	manualset3
153651	5	408311	13	NULL	NULL	0	NULL	53.63 mg/g	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Langmuir isotherm was used to describe the experimental adsorption , the maximum Cu2 + adsorption capacity of the kaolin/CA reached up to 53.63 mg/g .
	manualset3
153652	1	408312	13	NULL	NULL	0	NULL	Lepra Evaluation Project ( LEP )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Lepra Evaluation Project ( LEP ) , an epidemiological study of leprosy in northern Malai .
	manualset3
153653	2	408312	13	NULL	NULL	0	NULL	epidemiological study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Lepra Evaluation Project ( LEP ) , an epidemiological study of leprosy in northern Malai .
	manualset3
153654	3	408312	13	NULL	NULL	0	NULL	leprosy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The Lepra Evaluation Project ( LEP ) , an epidemiological study of leprosy in northern Malai .
	manualset3
153655	4	408312	13	NULL	NULL	0	NULL	northern Malai	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The Lepra Evaluation Project ( LEP ) , an epidemiological study of leprosy in northern Malai .
	manualset3
153656	1	408313	13	NULL	NULL	0	NULL	Lmo2 transcription factor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The Lmo2 transcription factor , a T-cell oncoprotein , is required for both hematopoiesis and angiogenesis .
	manualset3
153657	2	408313	13	NULL	NULL	0	NULL	 T-cell oncoprotein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The Lmo2 transcription factor , a T-cell oncoprotein , is required for both hematopoiesis and angiogenesis .
	manualset3
153658	3	408313	13	NULL	NULL	0	NULL	 hematopoiesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Lmo2 transcription factor , a T-cell oncoprotein , is required for both hematopoiesis and angiogenesis .
	manualset3
153659	4	408313	13	NULL	NULL	0	NULL	angiogenesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Lmo2 transcription factor , a T-cell oncoprotein , is required for both hematopoiesis and angiogenesis .
	manualset3
153660	1	408314	13	NULL	NULL	0	NULL	recombinant alpha 1-antitrypsin variant	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A recombinant alpha 1-antitrypsin variant which increased thermal stability was obtained from random mutagenesis followed by screening .
	manualset3
153661	2	408314	13	NULL	NULL	0	NULL	thermal stability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A recombinant alpha 1-antitrypsin variant which increased thermal stability was obtained from random mutagenesis followed by screening .
	manualset3
153662	3	408314	13	NULL	NULL	0	NULL	mutagenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A recombinant alpha 1-antitrypsin variant which increased thermal stability was obtained from random mutagenesis followed by screening .
	manualset3
153663	4	408314	13	NULL	NULL	0	NULL	screening	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A recombinant alpha 1-antitrypsin variant which increased thermal stability was obtained from random mutagenesis followed by screening .
	manualset3
153664	1	408315	13	NULL	NULL	0	NULL	Long	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Long and the Short of it : Gene and Environment Interactions During Early Cortical Development and Consequences for Long-Term Neurological Disease .
	manualset3
153665	2	408315	13	NULL	NULL	0	NULL	Short	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Long and the Short of it : Gene and Environment Interactions During Early Cortical Development and Consequences for Long-Term Neurological Disease .
	manualset3
153666	3	408315	13	NULL	NULL	0	NULL	Gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The Long and the Short of it : Gene and Environment Interactions During Early Cortical Development and Consequences for Long-Term Neurological Disease .
	manualset3
153667	4	408315	13	NULL	NULL	0	NULL	Environment	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The Long and the Short of it : Gene and Environment Interactions During Early Cortical Development and Consequences for Long-Term Neurological Disease .
	manualset3
153668	5	408315	13	NULL	NULL	0	NULL	Interactions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Long and the Short of it : Gene and Environment Interactions During Early Cortical Development and Consequences for Long-Term Neurological Disease .
	manualset3
153669	6	408315	13	NULL	NULL	0	NULL	Early Cortical Development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Long and the Short of it : Gene and Environment Interactions During Early Cortical Development and Consequences for Long-Term Neurological Disease .
	manualset3
153670	7	408315	13	NULL	NULL	0	NULL	Consequences	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Long and the Short of it : Gene and Environment Interactions During Early Cortical Development and Consequences for Long-Term Neurological Disease .
	manualset3
153671	8	408315	13	NULL	NULL	0	NULL	Long-Term Neurological Disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The Long and the Short of it : Gene and Environment Interactions During Early Cortical Development and Consequences for Long-Term Neurological Disease .
	manualset3
153672	1	408316	13	NULL	NULL	0	NULL	LungSign computerized system	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The LungSign computerized system was employed to scan cellular nuclei .
	manualset3
153673	2	408316	13	NULL	NULL	NULL	NULL	cellular nuclei	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The LungSign computerized system was employed to scan cellular nuclei .
	manualset3
153674	1	408317	13	NULL	NULL	0	NULL	M-component 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The M-component producing clone could be traced to extramedullary lymphoid tissue in myeloma but usually not in BMG .
	manualset3
153675	2	408317	13	NULL	NULL	NULL	NULL	clone	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The M-component producing clone could be traced to extramedullary lymphoid tissue in myeloma but usually not in BMG .
	manualset3
153676	3	408317	13	NULL	NULL	0	NULL	extramedullary lymphoid tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The M-component producing clone could be traced to extramedullary lymphoid tissue in myeloma but usually not in BMG .
	manualset3
153677	4	408317	13	NULL	NULL	0	NULL	myeloma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The M-component producing clone could be traced to extramedullary lymphoid tissue in myeloma but usually not in BMG .
	manualset3
153678	5	408317	13	NULL	NULL	0	NULL	BMG 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The M-component producing clone could be traced to extramedullary lymphoid tissue in myeloma but usually not in BMG .
	manualset3
153679	1	408318	13	NULL	NULL	0	NULL	M13 phage display system	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The M13 phage display system is a powerful technology for engineering proteins such as functional mutant proteins and peptides .
	manualset3
153680	2	408318	13	NULL	NULL	0	NULL	technology	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The M13 phage display system is a powerful technology for engineering proteins such as functional mutant proteins and peptides .
	manualset3
153681	3	408318	13	NULL	NULL	0	NULL	engineering proteins	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The M13 phage display system is a powerful technology for engineering proteins such as functional mutant proteins and peptides .
	manualset3
153682	4	408318	13	NULL	NULL	0	NULL	mutant proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The M13 phage display system is a powerful technology for engineering proteins such as functional mutant proteins and peptides .
	manualset3
153683	5	408318	13	NULL	NULL	0	NULL	peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The M13 phage display system is a powerful technology for engineering proteins such as functional mutant proteins and peptides .
	manualset3
153684	1	408319	13	NULL	NULL	NULL	NULL	MBO technique	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The MBO technique , involving the three primary functions of objective setting , objective using , and employee involvement , is described here in terms of both theory and practice .
	manualset3
153685	2	408319	13	NULL	NULL	0	NULL	primary functions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The MBO technique , involving the three primary functions of objective setting , objective using , and employee involvement , is described here in terms of both theory and practice .
	manualset3
153686	3	408319	13	NULL	NULL	0	NULL	objective setting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The MBO technique , involving the three primary functions of objective setting , objective using , and employee involvement , is described here in terms of both theory and practice .
	manualset3
153687	4	408319	13	NULL	NULL	0	NULL	objective using 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The MBO technique , involving the three primary functions of objective setting , objective using , and employee involvement , is described here in terms of both theory and practice .
	manualset3
153688	5	408319	13	NULL	NULL	0	NULL	employee involvement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The MBO technique , involving the three primary functions of objective setting , objective using , and employee involvement , is described here in terms of both theory and practice .
	manualset3
153689	6	408319	13	NULL	NULL	0	NULL	theory	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The MBO technique , involving the three primary functions of objective setting , objective using , and employee involvement , is described here in terms of both theory and practice .
	manualset3
153690	7	408319	13	NULL	NULL	0	NULL	practice 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The MBO technique , involving the three primary functions of objective setting , objective using , and employee involvement , is described here in terms of both theory and practice .
	manualset3
153691	1	408320	13	NULL	NULL	0	NULL	 MC assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The MC assay and detection by it of serum-blocking factors does not distinguish the effective anti-C3Hf lung tumor immune response of immunized C3Hf mice from the ineffective immune response of tumor-bearing ( A X C3Hf ) F1 and C3H mice .
	manualset3
153692	2	408320	13	NULL	NULL	0	NULL	detection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The MC assay and detection by it of serum-blocking factors does not distinguish the effective anti-C3Hf lung tumor immune response of immunized C3Hf mice from the ineffective immune response of tumor-bearing ( A X C3Hf ) F1 and C3H mice .
	manualset3
153693	3	408320	13	NULL	NULL	0	NULL	serum-blocking factors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The MC assay and detection by it of serum-blocking factors does not distinguish the effective anti-C3Hf lung tumor immune response of immunized C3Hf mice from the ineffective immune response of tumor-bearing ( A X C3Hf ) F1 and C3H mice .
	manualset3
153694	4	408320	13	NULL	NULL	0	NULL	anti-C3Hf lung tumor immune response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The MC assay and detection by it of serum-blocking factors does not distinguish the effective anti-C3Hf lung tumor immune response of immunized C3Hf mice from the ineffective immune response of tumor-bearing ( A X C3Hf ) F1 and C3H mice .
	manualset3
153695	5	408320	13	NULL	NULL	0	NULL	C3Hf mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The MC assay and detection by it of serum-blocking factors does not distinguish the effective anti-C3Hf lung tumor immune response of immunized C3Hf mice from the ineffective immune response of tumor-bearing ( A X C3Hf ) F1 and C3H mice .
	manualset3
153696	6	408320	13	NULL	NULL	0	NULL	 ineffective immune response 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The MC assay and detection by it of serum-blocking factors does not distinguish the effective anti-C3Hf lung tumor immune response of immunized C3Hf mice from the ineffective immune response of tumor-bearing ( A X C3Hf ) F1 and C3H mice .
	manualset3
153697	7	408320	13	NULL	NULL	0	NULL	tumor-bearing ( A X C3Hf ) F1 mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The MC assay and detection by it of serum-blocking factors does not distinguish the effective anti-C3Hf lung tumor immune response of immunized C3Hf mice from the ineffective immune response of tumor-bearing ( A X C3Hf ) F1 and C3H mice .
	manualset3
153698	8	408320	13	NULL	NULL	0	NULL	C3H mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The MC assay and detection by it of serum-blocking factors does not distinguish the effective anti-C3Hf lung tumor immune response of immunized C3Hf mice from the ineffective immune response of tumor-bearing ( A X C3Hf ) F1 and C3H mice .
	manualset3
153699	1	408321	13	NULL	NULL	0	NULL	MCV values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The MCV values will be too high if the instrument uses a high cell concentration , has a fixed lower threshold , no effective upper threshold and no edit facility .
	manualset3
153700	2	408321	13	NULL	NULL	0	NULL	 instrument	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The MCV values will be too high if the instrument uses a high cell concentration , has a fixed lower threshold , no effective upper threshold and no edit facility .
	manualset3
153701	3	408321	13	NULL	NULL	0	NULL	cell concentration 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The MCV values will be too high if the instrument uses a high cell concentration , has a fixed lower threshold , no effective upper threshold and no edit facility .
	manualset3
153702	4	408321	13	NULL	NULL	0	NULL	threshold	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The MCV values will be too high if the instrument uses a high cell concentration , has a fixed lower threshold , no effective upper threshold and no edit facility .
	manualset3
153703	5	408321	13	NULL	NULL	0	NULL	threshold	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The MCV values will be too high if the instrument uses a high cell concentration , has a fixed lower threshold , no effective upper threshold and no edit facility .
	manualset3
153704	6	408321	13	NULL	NULL	0	NULL	facility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The MCV values will be too high if the instrument uses a high cell concentration , has a fixed lower threshold , no effective upper threshold and no edit facility .
	manualset3
153705	1	408322	13	NULL	NULL	0	NULL	MDO1 gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The MDO1 gene encodes an unknown protein that is conserved in a wide variety of land plants .
	manualset3
153706	2	408322	13	NULL	NULL	0	NULL	protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The MDO1 gene encodes an unknown protein that is conserved in a wide variety of land plants .
	manualset3
153707	3	408322	13	NULL	NULL	0	NULL	 variety of land plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The MDO1 gene encodes an unknown protein that is conserved in a wide variety of land plants .
	manualset3
153708	1	408323	13	NULL	NULL	0	NULL	ME effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ME effect is usually observed in systems with peculiar couplings between a crystal lattice and a magnetic order .
	manualset3
153709	2	408323	13	NULL	NULL	0	NULL	systems	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ME effect is usually observed in systems with peculiar couplings between a crystal lattice and a magnetic order .
	manualset3
153710	3	408323	13	NULL	NULL	0	NULL	peculiar couplings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ME effect is usually observed in systems with peculiar couplings between a crystal lattice and a magnetic order .
	manualset3
153711	4	408323	13	NULL	NULL	0	NULL	crystal lattice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ME effect is usually observed in systems with peculiar couplings between a crystal lattice and a magnetic order .
	manualset3
153712	5	408323	13	NULL	NULL	0	NULL	magnetic order	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ME effect is usually observed in systems with peculiar couplings between a crystal lattice and a magnetic order .
	manualset3
153713	1	408324	13	NULL	NULL	0	NULL	MET proto-oncogene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The MET proto-oncogene encodes a transmembrane tyrosine kinase receptor that mediates multiple functions such as migration , cycling and survival by binding to hepatocyte growth factor ( HGF ) .
	manualset3
153714	2	408324	13	NULL	NULL	0	NULL	transmembrane tyrosine kinase receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The MET proto-oncogene encodes a transmembrane tyrosine kinase receptor that mediates multiple functions such as migration , cycling and survival by binding to hepatocyte growth factor ( HGF ) .
	manualset3
153715	3	408324	13	NULL	NULL	0	NULL	functions 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The MET proto-oncogene encodes a transmembrane tyrosine kinase receptor that mediates multiple functions such as migration , cycling and survival by binding to hepatocyte growth factor ( HGF ) .
	manualset3
153716	4	408324	13	NULL	NULL	0	NULL	 migration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The MET proto-oncogene encodes a transmembrane tyrosine kinase receptor that mediates multiple functions such as migration , cycling and survival by binding to hepatocyte growth factor ( HGF ) .
	manualset3
153717	5	408324	13	NULL	NULL	0	NULL	survival 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The MET proto-oncogene encodes a transmembrane tyrosine kinase receptor that mediates multiple functions such as migration , cycling and survival by binding to hepatocyte growth factor ( HGF ) .
	manualset3
153718	6	408324	13	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The MET proto-oncogene encodes a transmembrane tyrosine kinase receptor that mediates multiple functions such as migration , cycling and survival by binding to hepatocyte growth factor ( HGF ) .
	manualset3
153719	7	408324	13	NULL	NULL	0	NULL	hepatocyte growth factor ( HGF )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The MET proto-oncogene encodes a transmembrane tyrosine kinase receptor that mediates multiple functions such as migration , cycling and survival by binding to hepatocyte growth factor ( HGF ) .
	manualset3
153720	1	408325	13	NULL	NULL	0	NULL	 MIC90	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The MIC90 ( the minimum inhibitory concentration of an antibiotic necessary to inhibit the growth of 90 % of bacterial strains ) values of biapenem ( BIPM ) , meropenem ( MEPM ) , tazobactam/piperacillin ( TAZ/PIPC ) , sulbactam / cefoperazone ( SBT/CPZ ) , cefepime ( CFPM ) , ciprofloxacin ( CPFX ) , pazufloxacin ( PZFX ) , amikacin ( AMK ) and aztreonam ( AZT ) were found to be 265 , 512 , 256 , 512 , 512 , 64 , 128 , 128 and 128 microg/mL , respectively .
	manualset3
153721	2	408325	13	NULL	NULL	0	NULL	minimum inhibitory concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The MIC90 ( the minimum inhibitory concentration of an antibiotic necessary to inhibit the growth of 90 % of bacterial strains ) values of biapenem ( BIPM ) , meropenem ( MEPM ) , tazobactam/piperacillin ( TAZ/PIPC ) , sulbactam / cefoperazone ( SBT/CPZ ) , cefepime ( CFPM ) , ciprofloxacin ( CPFX ) , pazufloxacin ( PZFX ) , amikacin ( AMK ) and aztreonam ( AZT ) were found to be 265 , 512 , 256 , 512 , 512 , 64 , 128 , 128 and 128 microg/mL , respectively .
	manualset3
153722	3	408325	13	NULL	NULL	0	NULL	antibiotic	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The MIC90 ( the minimum inhibitory concentration of an antibiotic necessary to inhibit the growth of 90 % of bacterial strains ) values of biapenem ( BIPM ) , meropenem ( MEPM ) , tazobactam/piperacillin ( TAZ/PIPC ) , sulbactam / cefoperazone ( SBT/CPZ ) , cefepime ( CFPM ) , ciprofloxacin ( CPFX ) , pazufloxacin ( PZFX ) , amikacin ( AMK ) and aztreonam ( AZT ) were found to be 265 , 512 , 256 , 512 , 512 , 64 , 128 , 128 and 128 microg/mL , respectively .
	manualset3
153723	4	408325	13	NULL	NULL	0	NULL	growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The MIC90 ( the minimum inhibitory concentration of an antibiotic necessary to inhibit the growth of 90 % of bacterial strains ) values of biapenem ( BIPM ) , meropenem ( MEPM ) , tazobactam/piperacillin ( TAZ/PIPC ) , sulbactam / cefoperazone ( SBT/CPZ ) , cefepime ( CFPM ) , ciprofloxacin ( CPFX ) , pazufloxacin ( PZFX ) , amikacin ( AMK ) and aztreonam ( AZT ) were found to be 265 , 512 , 256 , 512 , 512 , 64 , 128 , 128 and 128 microg/mL , respectively .
	manualset3
153724	5	408325	13	NULL	NULL	0	NULL	90 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The MIC90 ( the minimum inhibitory concentration of an antibiotic necessary to inhibit the growth of 90 % of bacterial strains ) values of biapenem ( BIPM ) , meropenem ( MEPM ) , tazobactam/piperacillin ( TAZ/PIPC ) , sulbactam / cefoperazone ( SBT/CPZ ) , cefepime ( CFPM ) , ciprofloxacin ( CPFX ) , pazufloxacin ( PZFX ) , amikacin ( AMK ) and aztreonam ( AZT ) were found to be 265 , 512 , 256 , 512 , 512 , 64 , 128 , 128 and 128 microg/mL , respectively .
	manualset3
153725	6	408325	13	NULL	NULL	0	NULL	bacterial strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The MIC90 ( the minimum inhibitory concentration of an antibiotic necessary to inhibit the growth of 90 % of bacterial strains ) values of biapenem ( BIPM ) , meropenem ( MEPM ) , tazobactam/piperacillin ( TAZ/PIPC ) , sulbactam / cefoperazone ( SBT/CPZ ) , cefepime ( CFPM ) , ciprofloxacin ( CPFX ) , pazufloxacin ( PZFX ) , amikacin ( AMK ) and aztreonam ( AZT ) were found to be 265 , 512 , 256 , 512 , 512 , 64 , 128 , 128 and 128 microg/mL , respectively .
	manualset3
153726	7	408325	13	NULL	NULL	0	NULL	values 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The MIC90 ( the minimum inhibitory concentration of an antibiotic necessary to inhibit the growth of 90 % of bacterial strains ) values of biapenem ( BIPM ) , meropenem ( MEPM ) , tazobactam/piperacillin ( TAZ/PIPC ) , sulbactam / cefoperazone ( SBT/CPZ ) , cefepime ( CFPM ) , ciprofloxacin ( CPFX ) , pazufloxacin ( PZFX ) , amikacin ( AMK ) and aztreonam ( AZT ) were found to be 265 , 512 , 256 , 512 , 512 , 64 , 128 , 128 and 128 microg/mL , respectively .
	manualset3
153727	8	408325	13	NULL	NULL	0	NULL	biapenem ( BIPM )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The MIC90 ( the minimum inhibitory concentration of an antibiotic necessary to inhibit the growth of 90 % of bacterial strains ) values of biapenem ( BIPM ) , meropenem ( MEPM ) , tazobactam/piperacillin ( TAZ/PIPC ) , sulbactam / cefoperazone ( SBT/CPZ ) , cefepime ( CFPM ) , ciprofloxacin ( CPFX ) , pazufloxacin ( PZFX ) , amikacin ( AMK ) and aztreonam ( AZT ) were found to be 265 , 512 , 256 , 512 , 512 , 64 , 128 , 128 and 128 microg/mL , respectively .
	manualset3
153728	9	408325	13	NULL	NULL	0	NULL	meropenem ( MEPM )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The MIC90 ( the minimum inhibitory concentration of an antibiotic necessary to inhibit the growth of 90 % of bacterial strains ) values of biapenem ( BIPM ) , meropenem ( MEPM ) , tazobactam/piperacillin ( TAZ/PIPC ) , sulbactam / cefoperazone ( SBT/CPZ ) , cefepime ( CFPM ) , ciprofloxacin ( CPFX ) , pazufloxacin ( PZFX ) , amikacin ( AMK ) and aztreonam ( AZT ) were found to be 265 , 512 , 256 , 512 , 512 , 64 , 128 , 128 and 128 microg/mL , respectively .
	manualset3
153729	10	408325	13	NULL	NULL	0	NULL	tazobactam/piperacillin ( TAZ/PIPC )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The MIC90 ( the minimum inhibitory concentration of an antibiotic necessary to inhibit the growth of 90 % of bacterial strains ) values of biapenem ( BIPM ) , meropenem ( MEPM ) , tazobactam/piperacillin ( TAZ/PIPC ) , sulbactam / cefoperazone ( SBT/CPZ ) , cefepime ( CFPM ) , ciprofloxacin ( CPFX ) , pazufloxacin ( PZFX ) , amikacin ( AMK ) and aztreonam ( AZT ) were found to be 265 , 512 , 256 , 512 , 512 , 64 , 128 , 128 and 128 microg/mL , respectively .
	manualset3
153730	11	408325	13	NULL	NULL	0	NULL	sulbactam / cefoperazone ( SBT/CPZ ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The MIC90 ( the minimum inhibitory concentration of an antibiotic necessary to inhibit the growth of 90 % of bacterial strains ) values of biapenem ( BIPM ) , meropenem ( MEPM ) , tazobactam/piperacillin ( TAZ/PIPC ) , sulbactam / cefoperazone ( SBT/CPZ ) , cefepime ( CFPM ) , ciprofloxacin ( CPFX ) , pazufloxacin ( PZFX ) , amikacin ( AMK ) and aztreonam ( AZT ) were found to be 265 , 512 , 256 , 512 , 512 , 64 , 128 , 128 and 128 microg/mL , respectively .
	manualset3
153731	12	408325	13	NULL	NULL	0	NULL	cefepime ( CFPM )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The MIC90 ( the minimum inhibitory concentration of an antibiotic necessary to inhibit the growth of 90 % of bacterial strains ) values of biapenem ( BIPM ) , meropenem ( MEPM ) , tazobactam/piperacillin ( TAZ/PIPC ) , sulbactam / cefoperazone ( SBT/CPZ ) , cefepime ( CFPM ) , ciprofloxacin ( CPFX ) , pazufloxacin ( PZFX ) , amikacin ( AMK ) and aztreonam ( AZT ) were found to be 265 , 512 , 256 , 512 , 512 , 64 , 128 , 128 and 128 microg/mL , respectively .
	manualset3
153732	13	408325	13	NULL	NULL	0	NULL	ciprofloxacin ( CPFX )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The MIC90 ( the minimum inhibitory concentration of an antibiotic necessary to inhibit the growth of 90 % of bacterial strains ) values of biapenem ( BIPM ) , meropenem ( MEPM ) , tazobactam/piperacillin ( TAZ/PIPC ) , sulbactam / cefoperazone ( SBT/CPZ ) , cefepime ( CFPM ) , ciprofloxacin ( CPFX ) , pazufloxacin ( PZFX ) , amikacin ( AMK ) and aztreonam ( AZT ) were found to be 265 , 512 , 256 , 512 , 512 , 64 , 128 , 128 and 128 microg/mL , respectively .
	manualset3
153733	14	408325	13	NULL	NULL	0	NULL	pazufloxacin ( PZFX )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The MIC90 ( the minimum inhibitory concentration of an antibiotic necessary to inhibit the growth of 90 % of bacterial strains ) values of biapenem ( BIPM ) , meropenem ( MEPM ) , tazobactam/piperacillin ( TAZ/PIPC ) , sulbactam / cefoperazone ( SBT/CPZ ) , cefepime ( CFPM ) , ciprofloxacin ( CPFX ) , pazufloxacin ( PZFX ) , amikacin ( AMK ) and aztreonam ( AZT ) were found to be 265 , 512 , 256 , 512 , 512 , 64 , 128 , 128 and 128 microg/mL , respectively .
	manualset3
153734	15	408325	13	NULL	NULL	0	NULL	amikacin ( AMK )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The MIC90 ( the minimum inhibitory concentration of an antibiotic necessary to inhibit the growth of 90 % of bacterial strains ) values of biapenem ( BIPM ) , meropenem ( MEPM ) , tazobactam/piperacillin ( TAZ/PIPC ) , sulbactam / cefoperazone ( SBT/CPZ ) , cefepime ( CFPM ) , ciprofloxacin ( CPFX ) , pazufloxacin ( PZFX ) , amikacin ( AMK ) and aztreonam ( AZT ) were found to be 265 , 512 , 256 , 512 , 512 , 64 , 128 , 128 and 128 microg/mL , respectively .
	manualset3
153735	16	408325	13	NULL	NULL	0	NULL	aztreonam ( AZT )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The MIC90 ( the minimum inhibitory concentration of an antibiotic necessary to inhibit the growth of 90 % of bacterial strains ) values of biapenem ( BIPM ) , meropenem ( MEPM ) , tazobactam/piperacillin ( TAZ/PIPC ) , sulbactam / cefoperazone ( SBT/CPZ ) , cefepime ( CFPM ) , ciprofloxacin ( CPFX ) , pazufloxacin ( PZFX ) , amikacin ( AMK ) and aztreonam ( AZT ) were found to be 265 , 512 , 256 , 512 , 512 , 64 , 128 , 128 and 128 microg/mL , respectively .
	manualset3
153736	17	408325	13	NULL	NULL	0	NULL	265 microg/mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The MIC90 ( the minimum inhibitory concentration of an antibiotic necessary to inhibit the growth of 90 % of bacterial strains ) values of biapenem ( BIPM ) , meropenem ( MEPM ) , tazobactam/piperacillin ( TAZ/PIPC ) , sulbactam / cefoperazone ( SBT/CPZ ) , cefepime ( CFPM ) , ciprofloxacin ( CPFX ) , pazufloxacin ( PZFX ) , amikacin ( AMK ) and aztreonam ( AZT ) were found to be 265 , 512 , 256 , 512 , 512 , 64 , 128 , 128 and 128 microg/mL , respectively .
	manualset3
153737	18	408325	13	NULL	NULL	0	NULL	512 microg/mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The MIC90 ( the minimum inhibitory concentration of an antibiotic necessary to inhibit the growth of 90 % of bacterial strains ) values of biapenem ( BIPM ) , meropenem ( MEPM ) , tazobactam/piperacillin ( TAZ/PIPC ) , sulbactam / cefoperazone ( SBT/CPZ ) , cefepime ( CFPM ) , ciprofloxacin ( CPFX ) , pazufloxacin ( PZFX ) , amikacin ( AMK ) and aztreonam ( AZT ) were found to be 265 , 512 , 256 , 512 , 512 , 64 , 128 , 128 and 128 microg/mL , respectively .
	manualset3
153738	19	408325	13	NULL	NULL	0	NULL	256 microg/mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The MIC90 ( the minimum inhibitory concentration of an antibiotic necessary to inhibit the growth of 90 % of bacterial strains ) values of biapenem ( BIPM ) , meropenem ( MEPM ) , tazobactam/piperacillin ( TAZ/PIPC ) , sulbactam / cefoperazone ( SBT/CPZ ) , cefepime ( CFPM ) , ciprofloxacin ( CPFX ) , pazufloxacin ( PZFX ) , amikacin ( AMK ) and aztreonam ( AZT ) were found to be 265 , 512 , 256 , 512 , 512 , 64 , 128 , 128 and 128 microg/mL , respectively .
	manualset3
153739	20	408325	13	NULL	NULL	0	NULL	512 microg/mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The MIC90 ( the minimum inhibitory concentration of an antibiotic necessary to inhibit the growth of 90 % of bacterial strains ) values of biapenem ( BIPM ) , meropenem ( MEPM ) , tazobactam/piperacillin ( TAZ/PIPC ) , sulbactam / cefoperazone ( SBT/CPZ ) , cefepime ( CFPM ) , ciprofloxacin ( CPFX ) , pazufloxacin ( PZFX ) , amikacin ( AMK ) and aztreonam ( AZT ) were found to be 265 , 512 , 256 , 512 , 512 , 64 , 128 , 128 and 128 microg/mL , respectively .
	manualset3
153740	21	408325	13	NULL	NULL	0	NULL	512 microg/mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The MIC90 ( the minimum inhibitory concentration of an antibiotic necessary to inhibit the growth of 90 % of bacterial strains ) values of biapenem ( BIPM ) , meropenem ( MEPM ) , tazobactam/piperacillin ( TAZ/PIPC ) , sulbactam / cefoperazone ( SBT/CPZ ) , cefepime ( CFPM ) , ciprofloxacin ( CPFX ) , pazufloxacin ( PZFX ) , amikacin ( AMK ) and aztreonam ( AZT ) were found to be 265 , 512 , 256 , 512 , 512 , 64 , 128 , 128 and 128 microg/mL , respectively .
	manualset3
153741	22	408325	13	NULL	NULL	0	NULL	64 microg/mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The MIC90 ( the minimum inhibitory concentration of an antibiotic necessary to inhibit the growth of 90 % of bacterial strains ) values of biapenem ( BIPM ) , meropenem ( MEPM ) , tazobactam/piperacillin ( TAZ/PIPC ) , sulbactam / cefoperazone ( SBT/CPZ ) , cefepime ( CFPM ) , ciprofloxacin ( CPFX ) , pazufloxacin ( PZFX ) , amikacin ( AMK ) and aztreonam ( AZT ) were found to be 265 , 512 , 256 , 512 , 512 , 64 , 128 , 128 and 128 microg/mL , respectively .
	manualset3
153742	23	408325	13	NULL	NULL	0	NULL	128 microg/mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The MIC90 ( the minimum inhibitory concentration of an antibiotic necessary to inhibit the growth of 90 % of bacterial strains ) values of biapenem ( BIPM ) , meropenem ( MEPM ) , tazobactam/piperacillin ( TAZ/PIPC ) , sulbactam / cefoperazone ( SBT/CPZ ) , cefepime ( CFPM ) , ciprofloxacin ( CPFX ) , pazufloxacin ( PZFX ) , amikacin ( AMK ) and aztreonam ( AZT ) were found to be 265 , 512 , 256 , 512 , 512 , 64 , 128 , 128 and 128 microg/mL , respectively .
	manualset3
153743	24	408325	13	NULL	NULL	0	NULL	128 microg/mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The MIC90 ( the minimum inhibitory concentration of an antibiotic necessary to inhibit the growth of 90 % of bacterial strains ) values of biapenem ( BIPM ) , meropenem ( MEPM ) , tazobactam/piperacillin ( TAZ/PIPC ) , sulbactam / cefoperazone ( SBT/CPZ ) , cefepime ( CFPM ) , ciprofloxacin ( CPFX ) , pazufloxacin ( PZFX ) , amikacin ( AMK ) and aztreonam ( AZT ) were found to be 265 , 512 , 256 , 512 , 512 , 64 , 128 , 128 and 128 microg/mL , respectively .
	manualset3
153744	25	408325	13	NULL	NULL	0	NULL	128 microg/mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The MIC90 ( the minimum inhibitory concentration of an antibiotic necessary to inhibit the growth of 90 % of bacterial strains ) values of biapenem ( BIPM ) , meropenem ( MEPM ) , tazobactam/piperacillin ( TAZ/PIPC ) , sulbactam / cefoperazone ( SBT/CPZ ) , cefepime ( CFPM ) , ciprofloxacin ( CPFX ) , pazufloxacin ( PZFX ) , amikacin ( AMK ) and aztreonam ( AZT ) were found to be 265 , 512 , 256 , 512 , 512 , 64 , 128 , 128 and 128 microg/mL , respectively .
	manualset3
153745	1	408326	13	NULL	NULL	0	NULL	MP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The MP produced by KHOS cells did not react with the monoclonal anti-rat stromelysin antibody MC .
	manualset3
153746	2	408326	13	NULL	NULL	0	NULL	KHOS cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The MP produced by KHOS cells did not react with the monoclonal anti-rat stromelysin antibody MC .
	manualset3
153747	3	408326	13	NULL	NULL	0	NULL	 monoclonal anti-rat stromelysin antibody MC 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The MP produced by KHOS cells did not react with the monoclonal anti-rat stromelysin antibody MC .
	manualset3
153748	1	408327	13	NULL	NULL	0	NULL	 MRI appearance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The MRI appearance of the angiolipoma is reported here for the first time .
	manualset3
153749	2	408327	13	NULL	NULL	0	NULL	angiolipoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The MRI appearance of the angiolipoma is reported here for the first time .
	manualset3
153750	3	408327	13	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The MRI appearance of the angiolipoma is reported here for the first time .
	manualset3
153751	1	408328	13	NULL	NULL	0	NULL	MRSA 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The MRSA is considered a public health problem in neonatology because of its strong potential for dissemination in the wards associated with high rates of morbidity and mortality .
	manualset3
153752	2	408328	13	NULL	NULL	0	NULL	public health problem 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The MRSA is considered a public health problem in neonatology because of its strong potential for dissemination in the wards associated with high rates of morbidity and mortality .
	manualset3
153753	3	408328	13	NULL	NULL	0	NULL	neonatology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The MRSA is considered a public health problem in neonatology because of its strong potential for dissemination in the wards associated with high rates of morbidity and mortality .
	manualset3
153754	4	408328	13	NULL	NULL	0	NULL	potential for dissemination	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The MRSA is considered a public health problem in neonatology because of its strong potential for dissemination in the wards associated with high rates of morbidity and mortality .
	manualset3
153755	5	408328	13	NULL	NULL	0	NULL	wards	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The MRSA is considered a public health problem in neonatology because of its strong potential for dissemination in the wards associated with high rates of morbidity and mortality .
	manualset3
153756	6	408328	13	NULL	NULL	0	NULL	rates	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The MRSA is considered a public health problem in neonatology because of its strong potential for dissemination in the wards associated with high rates of morbidity and mortality .
	manualset3
153757	7	408328	13	NULL	NULL	0	NULL	 morbidity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The MRSA is considered a public health problem in neonatology because of its strong potential for dissemination in the wards associated with high rates of morbidity and mortality .
	manualset3
153758	8	408328	13	NULL	NULL	0	NULL	 mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The MRSA is considered a public health problem in neonatology because of its strong potential for dissemination in the wards associated with high rates of morbidity and mortality .
	manualset3
153759	1	408329	13	NULL	NULL	0	NULL	Mediator	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mediator is a large , multisubunit RNA polymerase II transcriptional regulator that was first identified in Saccharomyces cerevisiae as a factor required for responsiveness of Pol II and the general initiation factors to DNA binding transactivators .
	manualset3
153760	2	408329	13	NULL	NULL	0	NULL	large , multisubunit RNA polymerase II transcriptional regulator	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mediator is a large , multisubunit RNA polymerase II transcriptional regulator that was first identified in Saccharomyces cerevisiae as a factor required for responsiveness of Pol II and the general initiation factors to DNA binding transactivators .
	manualset3
153761	3	408329	13	NULL	NULL	0	NULL	Saccharomyces cerevisiae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mediator is a large , multisubunit RNA polymerase II transcriptional regulator that was first identified in Saccharomyces cerevisiae as a factor required for responsiveness of Pol II and the general initiation factors to DNA binding transactivators .
	manualset3
153762	4	408329	13	NULL	NULL	0	NULL	factor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mediator is a large , multisubunit RNA polymerase II transcriptional regulator that was first identified in Saccharomyces cerevisiae as a factor required for responsiveness of Pol II and the general initiation factors to DNA binding transactivators .
	manualset3
153763	5	408329	13	NULL	NULL	0	NULL	responsiveness 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mediator is a large , multisubunit RNA polymerase II transcriptional regulator that was first identified in Saccharomyces cerevisiae as a factor required for responsiveness of Pol II and the general initiation factors to DNA binding transactivators .
	manualset3
153764	6	408329	13	NULL	NULL	0	NULL	Pol II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mediator is a large , multisubunit RNA polymerase II transcriptional regulator that was first identified in Saccharomyces cerevisiae as a factor required for responsiveness of Pol II and the general initiation factors to DNA binding transactivators .
	manualset3
153765	7	408329	13	NULL	NULL	0	NULL	initiation factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mediator is a large , multisubunit RNA polymerase II transcriptional regulator that was first identified in Saccharomyces cerevisiae as a factor required for responsiveness of Pol II and the general initiation factors to DNA binding transactivators .
	manualset3
153766	8	408329	13	NULL	NULL	0	NULL	DNA binding transactivators	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mediator is a large , multisubunit RNA polymerase II transcriptional regulator that was first identified in Saccharomyces cerevisiae as a factor required for responsiveness of Pol II and the general initiation factors to DNA binding transactivators .
	manualset3
153767	1	408330	13	NULL	NULL	0	NULL	Mediterraneans	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mediterraneans had lower platelet counts ( 161 , 000 ( 89 , 000-290 , 000 ) / mul compared with 219 , 000 ( 148 , 000-323 , 000 ) / mul ) and higher arithmetic mean volumes ( 17.8 ( 10.8-29 .2 ) cu mum compared with 12.4 ( 9.9-15 .6 ) cu mum ) , while the individual lognormal platelet size distribution profiles were comparable ( geomatric standard deviations of 1.78 ( 1.60-1 .98 ) against 1.70 ( 1.54-1 .88 ) ) ; and the platelet biomass concentrations , given by count per microliter times mean volume times 10 - minus 7 and expressed as a volumetric percentage of whole blood , were almost identical ( 0.286 % ( 0.216 % -0.379 % ) against 0.272 % ( 0.201 % -0.367 % ) ) .
	manualset3
153768	2	408330	13	NULL	NULL	0	NULL	lower platelet counts	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mediterraneans had lower platelet counts ( 161 , 000 ( 89 , 000-290 , 000 ) / mul compared with 219 , 000 ( 148 , 000-323 , 000 ) / mul ) and higher arithmetic mean volumes ( 17.8 ( 10.8-29 .2 ) cu mum compared with 12.4 ( 9.9-15 .6 ) cu mum ) , while the individual lognormal platelet size distribution profiles were comparable ( geomatric standard deviations of 1.78 ( 1.60-1 .98 ) against 1.70 ( 1.54-1 .88 ) ) ; and the platelet biomass concentrations , given by count per microliter times mean volume times 10 - minus 7 and expressed as a volumetric percentage of whole blood , were almost identical ( 0.286 % ( 0.216 % -0.379 % ) against 0.272 % ( 0.201 % -0.367 % ) ) .
	manualset3
153769	3	408330	13	NULL	NULL	0	NULL	( 161 , 000 ( 89 , 000-290 , 000 ) / mul 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mediterraneans had lower platelet counts ( 161 , 000 ( 89 , 000-290 , 000 ) / mul compared with 219 , 000 ( 148 , 000-323 , 000 ) / mul ) and higher arithmetic mean volumes ( 17.8 ( 10.8-29 .2 ) cu mum compared with 12.4 ( 9.9-15 .6 ) cu mum ) , while the individual lognormal platelet size distribution profiles were comparable ( geomatric standard deviations of 1.78 ( 1.60-1 .98 ) against 1.70 ( 1.54-1 .88 ) ) ; and the platelet biomass concentrations , given by count per microliter times mean volume times 10 - minus 7 and expressed as a volumetric percentage of whole blood , were almost identical ( 0.286 % ( 0.216 % -0.379 % ) against 0.272 % ( 0.201 % -0.367 % ) ) .
	manualset3
153770	4	408330	13	NULL	NULL	0	NULL	219 , 000 ( 148 , 000-323 , 000 ) / mul ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mediterraneans had lower platelet counts ( 161 , 000 ( 89 , 000-290 , 000 ) / mul compared with 219 , 000 ( 148 , 000-323 , 000 ) / mul ) and higher arithmetic mean volumes ( 17.8 ( 10.8-29 .2 ) cu mum compared with 12.4 ( 9.9-15 .6 ) cu mum ) , while the individual lognormal platelet size distribution profiles were comparable ( geomatric standard deviations of 1.78 ( 1.60-1 .98 ) against 1.70 ( 1.54-1 .88 ) ) ; and the platelet biomass concentrations , given by count per microliter times mean volume times 10 - minus 7 and expressed as a volumetric percentage of whole blood , were almost identical ( 0.286 % ( 0.216 % -0.379 % ) against 0.272 % ( 0.201 % -0.367 % ) ) .
	manualset3
153771	5	408330	13	NULL	NULL	0	NULL	arithmetic mean volumes	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mediterraneans had lower platelet counts ( 161 , 000 ( 89 , 000-290 , 000 ) / mul compared with 219 , 000 ( 148 , 000-323 , 000 ) / mul ) and higher arithmetic mean volumes ( 17.8 ( 10.8-29 .2 ) cu mum compared with 12.4 ( 9.9-15 .6 ) cu mum ) , while the individual lognormal platelet size distribution profiles were comparable ( geomatric standard deviations of 1.78 ( 1.60-1 .98 ) against 1.70 ( 1.54-1 .88 ) ) ; and the platelet biomass concentrations , given by count per microliter times mean volume times 10 - minus 7 and expressed as a volumetric percentage of whole blood , were almost identical ( 0.286 % ( 0.216 % -0.379 % ) against 0.272 % ( 0.201 % -0.367 % ) ) .
	manualset3
153772	6	408330	13	NULL	NULL	0	NULL	( 17.8 ( 10.8-29 .2 ) cu mum	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mediterraneans had lower platelet counts ( 161 , 000 ( 89 , 000-290 , 000 ) / mul compared with 219 , 000 ( 148 , 000-323 , 000 ) / mul ) and higher arithmetic mean volumes ( 17.8 ( 10.8-29 .2 ) cu mum compared with 12.4 ( 9.9-15 .6 ) cu mum ) , while the individual lognormal platelet size distribution profiles were comparable ( geomatric standard deviations of 1.78 ( 1.60-1 .98 ) against 1.70 ( 1.54-1 .88 ) ) ; and the platelet biomass concentrations , given by count per microliter times mean volume times 10 - minus 7 and expressed as a volumetric percentage of whole blood , were almost identical ( 0.286 % ( 0.216 % -0.379 % ) against 0.272 % ( 0.201 % -0.367 % ) ) .
	manualset3
153773	7	408330	13	NULL	NULL	0	NULL	12.4 ( 9.9-15 .6 ) cu mum )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mediterraneans had lower platelet counts ( 161 , 000 ( 89 , 000-290 , 000 ) / mul compared with 219 , 000 ( 148 , 000-323 , 000 ) / mul ) and higher arithmetic mean volumes ( 17.8 ( 10.8-29 .2 ) cu mum compared with 12.4 ( 9.9-15 .6 ) cu mum ) , while the individual lognormal platelet size distribution profiles were comparable ( geomatric standard deviations of 1.78 ( 1.60-1 .98 ) against 1.70 ( 1.54-1 .88 ) ) ; and the platelet biomass concentrations , given by count per microliter times mean volume times 10 - minus 7 and expressed as a volumetric percentage of whole blood , were almost identical ( 0.286 % ( 0.216 % -0.379 % ) against 0.272 % ( 0.201 % -0.367 % ) ) .
	manualset3
153774	8	408330	13	NULL	NULL	0	NULL	platelet size distribution profiles	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mediterraneans had lower platelet counts ( 161 , 000 ( 89 , 000-290 , 000 ) / mul compared with 219 , 000 ( 148 , 000-323 , 000 ) / mul ) and higher arithmetic mean volumes ( 17.8 ( 10.8-29 .2 ) cu mum compared with 12.4 ( 9.9-15 .6 ) cu mum ) , while the individual lognormal platelet size distribution profiles were comparable ( geomatric standard deviations of 1.78 ( 1.60-1 .98 ) against 1.70 ( 1.54-1 .88 ) ) ; and the platelet biomass concentrations , given by count per microliter times mean volume times 10 - minus 7 and expressed as a volumetric percentage of whole blood , were almost identical ( 0.286 % ( 0.216 % -0.379 % ) against 0.272 % ( 0.201 % -0.367 % ) ) .
	manualset3
153775	9	408330	13	NULL	NULL	0	NULL	geomatric standard deviations 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mediterraneans had lower platelet counts ( 161 , 000 ( 89 , 000-290 , 000 ) / mul compared with 219 , 000 ( 148 , 000-323 , 000 ) / mul ) and higher arithmetic mean volumes ( 17.8 ( 10.8-29 .2 ) cu mum compared with 12.4 ( 9.9-15 .6 ) cu mum ) , while the individual lognormal platelet size distribution profiles were comparable ( geomatric standard deviations of 1.78 ( 1.60-1 .98 ) against 1.70 ( 1.54-1 .88 ) ) ; and the platelet biomass concentrations , given by count per microliter times mean volume times 10 - minus 7 and expressed as a volumetric percentage of whole blood , were almost identical ( 0.286 % ( 0.216 % -0.379 % ) against 0.272 % ( 0.201 % -0.367 % ) ) .
	manualset3
153776	10	408330	13	NULL	NULL	0	NULL	1.78 ( 1.60-1 .98 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mediterraneans had lower platelet counts ( 161 , 000 ( 89 , 000-290 , 000 ) / mul compared with 219 , 000 ( 148 , 000-323 , 000 ) / mul ) and higher arithmetic mean volumes ( 17.8 ( 10.8-29 .2 ) cu mum compared with 12.4 ( 9.9-15 .6 ) cu mum ) , while the individual lognormal platelet size distribution profiles were comparable ( geomatric standard deviations of 1.78 ( 1.60-1 .98 ) against 1.70 ( 1.54-1 .88 ) ) ; and the platelet biomass concentrations , given by count per microliter times mean volume times 10 - minus 7 and expressed as a volumetric percentage of whole blood , were almost identical ( 0.286 % ( 0.216 % -0.379 % ) against 0.272 % ( 0.201 % -0.367 % ) ) .
	manualset3
153777	11	408330	13	NULL	NULL	0	NULL	1.70 ( 1.54-1 .88 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mediterraneans had lower platelet counts ( 161 , 000 ( 89 , 000-290 , 000 ) / mul compared with 219 , 000 ( 148 , 000-323 , 000 ) / mul ) and higher arithmetic mean volumes ( 17.8 ( 10.8-29 .2 ) cu mum compared with 12.4 ( 9.9-15 .6 ) cu mum ) , while the individual lognormal platelet size distribution profiles were comparable ( geomatric standard deviations of 1.78 ( 1.60-1 .98 ) against 1.70 ( 1.54-1 .88 ) ) ; and the platelet biomass concentrations , given by count per microliter times mean volume times 10 - minus 7 and expressed as a volumetric percentage of whole blood , were almost identical ( 0.286 % ( 0.216 % -0.379 % ) against 0.272 % ( 0.201 % -0.367 % ) ) .
	manualset3
153778	12	408330	13	NULL	NULL	0	NULL	platelet biomass concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mediterraneans had lower platelet counts ( 161 , 000 ( 89 , 000-290 , 000 ) / mul compared with 219 , 000 ( 148 , 000-323 , 000 ) / mul ) and higher arithmetic mean volumes ( 17.8 ( 10.8-29 .2 ) cu mum compared with 12.4 ( 9.9-15 .6 ) cu mum ) , while the individual lognormal platelet size distribution profiles were comparable ( geomatric standard deviations of 1.78 ( 1.60-1 .98 ) against 1.70 ( 1.54-1 .88 ) ) ; and the platelet biomass concentrations , given by count per microliter times mean volume times 10 - minus 7 and expressed as a volumetric percentage of whole blood , were almost identical ( 0.286 % ( 0.216 % -0.379 % ) against 0.272 % ( 0.201 % -0.367 % ) ) .
	manualset3
153779	13	408330	13	NULL	NULL	0	NULL	count per microliter times mean volume times 10 - minus 7	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mediterraneans had lower platelet counts ( 161 , 000 ( 89 , 000-290 , 000 ) / mul compared with 219 , 000 ( 148 , 000-323 , 000 ) / mul ) and higher arithmetic mean volumes ( 17.8 ( 10.8-29 .2 ) cu mum compared with 12.4 ( 9.9-15 .6 ) cu mum ) , while the individual lognormal platelet size distribution profiles were comparable ( geomatric standard deviations of 1.78 ( 1.60-1 .98 ) against 1.70 ( 1.54-1 .88 ) ) ; and the platelet biomass concentrations , given by count per microliter times mean volume times 10 - minus 7 and expressed as a volumetric percentage of whole blood , were almost identical ( 0.286 % ( 0.216 % -0.379 % ) against 0.272 % ( 0.201 % -0.367 % ) ) .
	manualset3
153780	14	408330	13	NULL	NULL	0	NULL	volumetric percentage of whole blood	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mediterraneans had lower platelet counts ( 161 , 000 ( 89 , 000-290 , 000 ) / mul compared with 219 , 000 ( 148 , 000-323 , 000 ) / mul ) and higher arithmetic mean volumes ( 17.8 ( 10.8-29 .2 ) cu mum compared with 12.4 ( 9.9-15 .6 ) cu mum ) , while the individual lognormal platelet size distribution profiles were comparable ( geomatric standard deviations of 1.78 ( 1.60-1 .98 ) against 1.70 ( 1.54-1 .88 ) ) ; and the platelet biomass concentrations , given by count per microliter times mean volume times 10 - minus 7 and expressed as a volumetric percentage of whole blood , were almost identical ( 0.286 % ( 0.216 % -0.379 % ) against 0.272 % ( 0.201 % -0.367 % ) ) .
	manualset3
153781	15	408330	13	NULL	NULL	0	NULL	0.286 % ( 0.216 % -0.379 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mediterraneans had lower platelet counts ( 161 , 000 ( 89 , 000-290 , 000 ) / mul compared with 219 , 000 ( 148 , 000-323 , 000 ) / mul ) and higher arithmetic mean volumes ( 17.8 ( 10.8-29 .2 ) cu mum compared with 12.4 ( 9.9-15 .6 ) cu mum ) , while the individual lognormal platelet size distribution profiles were comparable ( geomatric standard deviations of 1.78 ( 1.60-1 .98 ) against 1.70 ( 1.54-1 .88 ) ) ; and the platelet biomass concentrations , given by count per microliter times mean volume times 10 - minus 7 and expressed as a volumetric percentage of whole blood , were almost identical ( 0.286 % ( 0.216 % -0.379 % ) against 0.272 % ( 0.201 % -0.367 % ) ) .
	manualset3
153782	16	408330	13	NULL	NULL	0	NULL	 0.272 % ( 0.201 % -0.367 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mediterraneans had lower platelet counts ( 161 , 000 ( 89 , 000-290 , 000 ) / mul compared with 219 , 000 ( 148 , 000-323 , 000 ) / mul ) and higher arithmetic mean volumes ( 17.8 ( 10.8-29 .2 ) cu mum compared with 12.4 ( 9.9-15 .6 ) cu mum ) , while the individual lognormal platelet size distribution profiles were comparable ( geomatric standard deviations of 1.78 ( 1.60-1 .98 ) against 1.70 ( 1.54-1 .88 ) ) ; and the platelet biomass concentrations , given by count per microliter times mean volume times 10 - minus 7 and expressed as a volumetric percentage of whole blood , were almost identical ( 0.286 % ( 0.216 % -0.379 % ) against 0.272 % ( 0.201 % -0.367 % ) ) .
	manualset3
153783	1	408331	13	NULL	NULL	0	NULL	Mental Health Act 2007	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mental Health Act 2007 introduced an amendment to the Mental Capacity Act 2005 that authorizes the deprivation of liberty of a person who lacks decision-making capacity in a care home or hospital where this is necessary to protect them from harm .
	manualset3
153784	2	408331	13	NULL	NULL	0	NULL	amendment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mental Health Act 2007 introduced an amendment to the Mental Capacity Act 2005 that authorizes the deprivation of liberty of a person who lacks decision-making capacity in a care home or hospital where this is necessary to protect them from harm .
	manualset3
153785	3	408331	13	NULL	NULL	0	NULL	Mental Capacity Act 2005 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mental Health Act 2007 introduced an amendment to the Mental Capacity Act 2005 that authorizes the deprivation of liberty of a person who lacks decision-making capacity in a care home or hospital where this is necessary to protect them from harm .
	manualset3
153786	4	408331	13	NULL	NULL	0	NULL	deprivation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mental Health Act 2007 introduced an amendment to the Mental Capacity Act 2005 that authorizes the deprivation of liberty of a person who lacks decision-making capacity in a care home or hospital where this is necessary to protect them from harm .
	manualset3
153787	5	408331	13	NULL	NULL	0	NULL	liberty 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mental Health Act 2007 introduced an amendment to the Mental Capacity Act 2005 that authorizes the deprivation of liberty of a person who lacks decision-making capacity in a care home or hospital where this is necessary to protect them from harm .
	manualset3
153788	6	408331	13	NULL	NULL	0	NULL	person	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mental Health Act 2007 introduced an amendment to the Mental Capacity Act 2005 that authorizes the deprivation of liberty of a person who lacks decision-making capacity in a care home or hospital where this is necessary to protect them from harm .
	manualset3
153789	7	408331	13	NULL	NULL	0	NULL	decision-making capacity	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mental Health Act 2007 introduced an amendment to the Mental Capacity Act 2005 that authorizes the deprivation of liberty of a person who lacks decision-making capacity in a care home or hospital where this is necessary to protect them from harm .
	manualset3
153790	8	408331	13	NULL	NULL	0	NULL	care home	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mental Health Act 2007 introduced an amendment to the Mental Capacity Act 2005 that authorizes the deprivation of liberty of a person who lacks decision-making capacity in a care home or hospital where this is necessary to protect them from harm .
	manualset3
153791	9	408331	13	NULL	NULL	0	NULL	hospital 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mental Health Act 2007 introduced an amendment to the Mental Capacity Act 2005 that authorizes the deprivation of liberty of a person who lacks decision-making capacity in a care home or hospital where this is necessary to protect them from harm .
	manualset3
153792	10	408331	13	NULL	NULL	0	NULL	harm	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mental Health Act 2007 introduced an amendment to the Mental Capacity Act 2005 that authorizes the deprivation of liberty of a person who lacks decision-making capacity in a care home or hospital where this is necessary to protect them from harm .
	manualset3
153793	1	408332	13	NULL	NULL	0	NULL	 reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A reduction of ST segment greater than 22 mm is characterized by decrease of sensitivity ( 40 % ) but with a considerable increase of specificity ( 96 % ) .
	manualset3
153794	2	408332	13	NULL	NULL	0	NULL	ST segment	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A reduction of ST segment greater than 22 mm is characterized by decrease of sensitivity ( 40 % ) but with a considerable increase of specificity ( 96 % ) .
	manualset3
153795	3	408332	13	NULL	NULL	0	NULL	22 mm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A reduction of ST segment greater than 22 mm is characterized by decrease of sensitivity ( 40 % ) but with a considerable increase of specificity ( 96 % ) .
	manualset3
153796	4	408332	13	NULL	NULL	0	NULL	decrease 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A reduction of ST segment greater than 22 mm is characterized by decrease of sensitivity ( 40 % ) but with a considerable increase of specificity ( 96 % ) .
	manualset3
153797	5	408332	13	NULL	NULL	0	NULL	sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A reduction of ST segment greater than 22 mm is characterized by decrease of sensitivity ( 40 % ) but with a considerable increase of specificity ( 96 % ) .
	manualset3
153798	6	408332	13	NULL	NULL	0	NULL	( 40 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A reduction of ST segment greater than 22 mm is characterized by decrease of sensitivity ( 40 % ) but with a considerable increase of specificity ( 96 % ) .
	manualset3
153799	7	408332	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A reduction of ST segment greater than 22 mm is characterized by decrease of sensitivity ( 40 % ) but with a considerable increase of specificity ( 96 % ) .
	manualset3
153800	8	408332	13	NULL	NULL	0	NULL	specificity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A reduction of ST segment greater than 22 mm is characterized by decrease of sensitivity ( 40 % ) but with a considerable increase of specificity ( 96 % ) .
	manualset3
153801	9	408332	13	NULL	NULL	0	NULL	96 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A reduction of ST segment greater than 22 mm is characterized by decrease of sensitivity ( 40 % ) but with a considerable increase of specificity ( 96 % ) .
	manualset3
153802	1	408333	13	NULL	NULL	0	NULL	Michaelis constant 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The Michaelis constant for 3 , 6-dichlorobenzene cis-dihydrodiol ( 210 microM ) was lower than for benzene cis-dihydrodiol ( 780 microM ) , while the specific activity with benzene cis-dihydrodiol ( 63 units / mg ) was higher than with 3 , 6-dichlorobenzene cis-dihydrodiol ( 32 units/mg ) .
	manualset3
153803	2	408333	13	NULL	NULL	0	NULL	3 , 6-dichlorobenzene cis-dihydrodiol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The Michaelis constant for 3 , 6-dichlorobenzene cis-dihydrodiol ( 210 microM ) was lower than for benzene cis-dihydrodiol ( 780 microM ) , while the specific activity with benzene cis-dihydrodiol ( 63 units / mg ) was higher than with 3 , 6-dichlorobenzene cis-dihydrodiol ( 32 units/mg ) .
	manualset3
153804	3	408333	13	NULL	NULL	0	NULL	210 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Michaelis constant for 3 , 6-dichlorobenzene cis-dihydrodiol ( 210 microM ) was lower than for benzene cis-dihydrodiol ( 780 microM ) , while the specific activity with benzene cis-dihydrodiol ( 63 units / mg ) was higher than with 3 , 6-dichlorobenzene cis-dihydrodiol ( 32 units/mg ) .
	manualset3
153805	4	408333	13	NULL	NULL	0	NULL	benzene cis-dihydrodiol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The Michaelis constant for 3 , 6-dichlorobenzene cis-dihydrodiol ( 210 microM ) was lower than for benzene cis-dihydrodiol ( 780 microM ) , while the specific activity with benzene cis-dihydrodiol ( 63 units / mg ) was higher than with 3 , 6-dichlorobenzene cis-dihydrodiol ( 32 units/mg ) .
	manualset3
153806	5	408333	13	NULL	NULL	0	NULL	780 microM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Michaelis constant for 3 , 6-dichlorobenzene cis-dihydrodiol ( 210 microM ) was lower than for benzene cis-dihydrodiol ( 780 microM ) , while the specific activity with benzene cis-dihydrodiol ( 63 units / mg ) was higher than with 3 , 6-dichlorobenzene cis-dihydrodiol ( 32 units/mg ) .
	manualset3
153807	6	408333	13	NULL	NULL	0	NULL	specific activity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Michaelis constant for 3 , 6-dichlorobenzene cis-dihydrodiol ( 210 microM ) was lower than for benzene cis-dihydrodiol ( 780 microM ) , while the specific activity with benzene cis-dihydrodiol ( 63 units / mg ) was higher than with 3 , 6-dichlorobenzene cis-dihydrodiol ( 32 units/mg ) .
	manualset3
153808	7	408333	13	NULL	NULL	0	NULL	benzene cis-dihydrodiol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The Michaelis constant for 3 , 6-dichlorobenzene cis-dihydrodiol ( 210 microM ) was lower than for benzene cis-dihydrodiol ( 780 microM ) , while the specific activity with benzene cis-dihydrodiol ( 63 units / mg ) was higher than with 3 , 6-dichlorobenzene cis-dihydrodiol ( 32 units/mg ) .
	manualset3
153809	8	408333	13	NULL	NULL	0	NULL	63 units / mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Michaelis constant for 3 , 6-dichlorobenzene cis-dihydrodiol ( 210 microM ) was lower than for benzene cis-dihydrodiol ( 780 microM ) , while the specific activity with benzene cis-dihydrodiol ( 63 units / mg ) was higher than with 3 , 6-dichlorobenzene cis-dihydrodiol ( 32 units/mg ) .
	manualset3
153810	9	408333	13	NULL	NULL	0	NULL	3 , 6-dichlorobenzene cis-dihydrodiol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The Michaelis constant for 3 , 6-dichlorobenzene cis-dihydrodiol ( 210 microM ) was lower than for benzene cis-dihydrodiol ( 780 microM ) , while the specific activity with benzene cis-dihydrodiol ( 63 units / mg ) was higher than with 3 , 6-dichlorobenzene cis-dihydrodiol ( 32 units/mg ) .
	manualset3
153811	10	408333	13	NULL	NULL	0	NULL	32 units/mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Michaelis constant for 3 , 6-dichlorobenzene cis-dihydrodiol ( 210 microM ) was lower than for benzene cis-dihydrodiol ( 780 microM ) , while the specific activity with benzene cis-dihydrodiol ( 63 units / mg ) was higher than with 3 , 6-dichlorobenzene cis-dihydrodiol ( 32 units/mg ) .
	manualset3
153812	1	408334	13	NULL	NULL	0	NULL	MixAlco process	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The MixAlco process employs a mixed culture of acid-forming microorganisms to convert biomass to carboxylate salts , which are concentrated via vapor-compression evaporation and subsequently chemically converted to other chemical and fuel products .
	manualset3
153813	2	408334	13	NULL	NULL	0	NULL	culture	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The MixAlco process employs a mixed culture of acid-forming microorganisms to convert biomass to carboxylate salts , which are concentrated via vapor-compression evaporation and subsequently chemically converted to other chemical and fuel products .
	manualset3
153814	3	408334	13	NULL	NULL	0	NULL	microorganisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The MixAlco process employs a mixed culture of acid-forming microorganisms to convert biomass to carboxylate salts , which are concentrated via vapor-compression evaporation and subsequently chemically converted to other chemical and fuel products .
	manualset3
153815	4	408334	13	NULL	NULL	0	NULL	biomass	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The MixAlco process employs a mixed culture of acid-forming microorganisms to convert biomass to carboxylate salts , which are concentrated via vapor-compression evaporation and subsequently chemically converted to other chemical and fuel products .
	manualset3
153816	5	408334	13	NULL	NULL	0	NULL	carboxylate salts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The MixAlco process employs a mixed culture of acid-forming microorganisms to convert biomass to carboxylate salts , which are concentrated via vapor-compression evaporation and subsequently chemically converted to other chemical and fuel products .
	manualset3
153817	6	408334	13	NULL	NULL	0	NULL	vapor-compression evaporation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The MixAlco process employs a mixed culture of acid-forming microorganisms to convert biomass to carboxylate salts , which are concentrated via vapor-compression evaporation and subsequently chemically converted to other chemical and fuel products .
	manualset3
153818	7	408334	13	NULL	NULL	0	NULL	chemical products	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The MixAlco process employs a mixed culture of acid-forming microorganisms to convert biomass to carboxylate salts , which are concentrated via vapor-compression evaporation and subsequently chemically converted to other chemical and fuel products .
	manualset3
153819	8	408334	13	NULL	NULL	0	NULL	fuel products 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The MixAlco process employs a mixed culture of acid-forming microorganisms to convert biomass to carboxylate salts , which are concentrated via vapor-compression evaporation and subsequently chemically converted to other chemical and fuel products .
	manualset3
153820	1	408335	13	NULL	NULL	0	NULL	Mongolian Ministry of Health	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mongolian Ministry of Health asked the World Health Organization ( WHO ) and the United Nations Children 's Fund ( UNICEF ) for assistance in assessing the nutritional effects of the 2000-2001 dzud on children aged 6-59 months .
	manualset3
153821	2	408335	13	NULL	NULL	NULL	NULL	World Health Organization ( WHO )	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The Mongolian Ministry of Health asked the World Health Organization ( WHO ) and the United Nations Children 's Fund ( UNICEF ) for assistance in assessing the nutritional effects of the 2000-2001 dzud on children aged 6-59 months .
	manualset3
153822	3	408335	13	NULL	NULL	0	NULL	United Nations Children 's Fund ( UNICEF ) 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mongolian Ministry of Health asked the World Health Organization ( WHO ) and the United Nations Children 's Fund ( UNICEF ) for assistance in assessing the nutritional effects of the 2000-2001 dzud on children aged 6-59 months .
	manualset3
153823	4	408335	13	NULL	NULL	0	NULL	assistance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mongolian Ministry of Health asked the World Health Organization ( WHO ) and the United Nations Children 's Fund ( UNICEF ) for assistance in assessing the nutritional effects of the 2000-2001 dzud on children aged 6-59 months .
	manualset3
153824	5	408335	13	NULL	NULL	0	NULL	nutritional effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mongolian Ministry of Health asked the World Health Organization ( WHO ) and the United Nations Children 's Fund ( UNICEF ) for assistance in assessing the nutritional effects of the 2000-2001 dzud on children aged 6-59 months .
	manualset3
153825	6	408335	13	NULL	NULL	0	NULL	2000-2001 dzud	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mongolian Ministry of Health asked the World Health Organization ( WHO ) and the United Nations Children 's Fund ( UNICEF ) for assistance in assessing the nutritional effects of the 2000-2001 dzud on children aged 6-59 months .
	manualset3
153826	7	408335	13	NULL	NULL	0	NULL	children aged 6-59 months	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The Mongolian Ministry of Health asked the World Health Organization ( WHO ) and the United Nations Children 's Fund ( UNICEF ) for assistance in assessing the nutritional effects of the 2000-2001 dzud on children aged 6-59 months .
	manualset3
153827	1	408336	13	NULL	NULL	0	NULL	Msh6-S cyclin fusion 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Msh6-S cyclin fusion was proficient for suppressing mutations at three loci that replicate at mid-S phase , whereas the Msh6-G2 / M cyclin fusion was defective .
	manualset3
153828	2	408336	13	NULL	NULL	0	NULL	mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Msh6-S cyclin fusion was proficient for suppressing mutations at three loci that replicate at mid-S phase , whereas the Msh6-G2 / M cyclin fusion was defective .
	manualset3
153829	3	408336	13	NULL	NULL	0	NULL	three loci 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Msh6-S cyclin fusion was proficient for suppressing mutations at three loci that replicate at mid-S phase , whereas the Msh6-G2 / M cyclin fusion was defective .
	manualset3
153830	4	408336	13	NULL	NULL	0	NULL	mid-S phase	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The Msh6-S cyclin fusion was proficient for suppressing mutations at three loci that replicate at mid-S phase , whereas the Msh6-G2 / M cyclin fusion was defective .
	manualset3
153831	5	408336	13	NULL	NULL	0	NULL	Msh6-G2 / M cyclin fusion 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Msh6-S cyclin fusion was proficient for suppressing mutations at three loci that replicate at mid-S phase , whereas the Msh6-G2 / M cyclin fusion was defective .
	manualset3
153832	1	408337	13	NULL	NULL	0	NULL	N-methyl-D-aspartate receptor blocker MK-801	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The N-methyl-D-aspartate receptor blocker MK-801 prevents the facilitatory effects of naloxone and epinephrine on retention of inhibitory avoidance task in rats .
	manualset3
153833	2	408337	13	NULL	NULL	0	NULL	facilitatory effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The N-methyl-D-aspartate receptor blocker MK-801 prevents the facilitatory effects of naloxone and epinephrine on retention of inhibitory avoidance task in rats .
	manualset3
153834	3	408337	13	NULL	NULL	0	NULL	naloxone 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The N-methyl-D-aspartate receptor blocker MK-801 prevents the facilitatory effects of naloxone and epinephrine on retention of inhibitory avoidance task in rats .
	manualset3
153835	4	408337	13	NULL	NULL	0	NULL	epinephrine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The N-methyl-D-aspartate receptor blocker MK-801 prevents the facilitatory effects of naloxone and epinephrine on retention of inhibitory avoidance task in rats .
	manualset3
153836	5	408337	13	NULL	NULL	0	NULL	avoidance task 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The N-methyl-D-aspartate receptor blocker MK-801 prevents the facilitatory effects of naloxone and epinephrine on retention of inhibitory avoidance task in rats .
	manualset3
153837	6	408337	13	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The N-methyl-D-aspartate receptor blocker MK-801 prevents the facilitatory effects of naloxone and epinephrine on retention of inhibitory avoidance task in rats .
	manualset3
153838	7	408337	13	NULL	NULL	0	NULL	retention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The N-methyl-D-aspartate receptor blocker MK-801 prevents the facilitatory effects of naloxone and epinephrine on retention of inhibitory avoidance task in rats .
	manualset3
153839	1	408338	13	NULL	NULL	0	NULL	N-terminal 5 ' -3 ' exonuclease domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The N-terminal 5 ' -3 ' exonuclease domain and the C-terminal polymerase domain show 31 and 46 % identity , respectively , with the corresponding E. coli domains and all sequence motifs associated with these two enzymatic activities also are conserved .
	manualset3
153840	2	408338	13	NULL	NULL	0	NULL	C-terminal polymerase domain 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The N-terminal 5 ' -3 ' exonuclease domain and the C-terminal polymerase domain show 31 and 46 % identity , respectively , with the corresponding E. coli domains and all sequence motifs associated with these two enzymatic activities also are conserved .
	manualset3
153841	3	408338	13	NULL	NULL	0	NULL	31 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The N-terminal 5 ' -3 ' exonuclease domain and the C-terminal polymerase domain show 31 and 46 % identity , respectively , with the corresponding E. coli domains and all sequence motifs associated with these two enzymatic activities also are conserved .
	manualset3
153842	4	408338	13	NULL	NULL	0	NULL	46 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The N-terminal 5 ' -3 ' exonuclease domain and the C-terminal polymerase domain show 31 and 46 % identity , respectively , with the corresponding E. coli domains and all sequence motifs associated with these two enzymatic activities also are conserved .
	manualset3
153843	5	408338	13	NULL	NULL	0	NULL	identity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The N-terminal 5 ' -3 ' exonuclease domain and the C-terminal polymerase domain show 31 and 46 % identity , respectively , with the corresponding E. coli domains and all sequence motifs associated with these two enzymatic activities also are conserved .
	manualset3
153844	6	408338	13	NULL	NULL	0	NULL	E. coli domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The N-terminal 5 ' -3 ' exonuclease domain and the C-terminal polymerase domain show 31 and 46 % identity , respectively , with the corresponding E. coli domains and all sequence motifs associated with these two enzymatic activities also are conserved .
	manualset3
153845	7	408338	13	NULL	NULL	0	NULL	sequence motifs 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The N-terminal 5 ' -3 ' exonuclease domain and the C-terminal polymerase domain show 31 and 46 % identity , respectively , with the corresponding E. coli domains and all sequence motifs associated with these two enzymatic activities also are conserved .
	manualset3
153846	8	408338	13	NULL	NULL	0	NULL	two enzymatic activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The N-terminal 5 ' -3 ' exonuclease domain and the C-terminal polymerase domain show 31 and 46 % identity , respectively , with the corresponding E. coli domains and all sequence motifs associated with these two enzymatic activities also are conserved .
	manualset3
153847	1	408339	13	NULL	NULL	0	NULL	N-terminal DNA-binding domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The N-terminal DNA-binding domain of the multidrug transporter activation protein ( MtaN ) was crystallized by the hanging-drop vapour-diffusion method using lithium chloride as a precipitant .
	manualset3
153848	2	408339	13	NULL	NULL	0	NULL	multidrug transporter activation protein ( MtaN )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The N-terminal DNA-binding domain of the multidrug transporter activation protein ( MtaN ) was crystallized by the hanging-drop vapour-diffusion method using lithium chloride as a precipitant .
	manualset3
153849	3	408339	13	NULL	NULL	0	NULL	hanging-drop vapour-diffusion method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The N-terminal DNA-binding domain of the multidrug transporter activation protein ( MtaN ) was crystallized by the hanging-drop vapour-diffusion method using lithium chloride as a precipitant .
	manualset3
153850	4	408339	13	NULL	NULL	0	NULL	lithium chloride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The N-terminal DNA-binding domain of the multidrug transporter activation protein ( MtaN ) was crystallized by the hanging-drop vapour-diffusion method using lithium chloride as a precipitant .
	manualset3
153851	5	408339	13	NULL	NULL	0	NULL	 precipitant	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The N-terminal DNA-binding domain of the multidrug transporter activation protein ( MtaN ) was crystallized by the hanging-drop vapour-diffusion method using lithium chloride as a precipitant .
	manualset3
153852	1	408340	13	NULL	NULL	0	NULL	 N-terminal region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The N-terminal region in rat TBP1 , TBP7 , and SUG1 contains a heptad repeat of hydrophobic amino acids reminiscent of a leucine zipper .
	manualset3
153853	2	408340	13	NULL	NULL	0	NULL	rat TBP1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The N-terminal region in rat TBP1 , TBP7 , and SUG1 contains a heptad repeat of hydrophobic amino acids reminiscent of a leucine zipper .
	manualset3
153854	3	408340	13	NULL	NULL	0	NULL	TBP7 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The N-terminal region in rat TBP1 , TBP7 , and SUG1 contains a heptad repeat of hydrophobic amino acids reminiscent of a leucine zipper .
	manualset3
153855	4	408340	13	NULL	NULL	0	NULL	SUG1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The N-terminal region in rat TBP1 , TBP7 , and SUG1 contains a heptad repeat of hydrophobic amino acids reminiscent of a leucine zipper .
	manualset3
153856	5	408340	13	NULL	NULL	NULL	NULL	heptad repeat of hydrophobic amino acids 	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The N-terminal region in rat TBP1 , TBP7 , and SUG1 contains a heptad repeat of hydrophobic amino acids reminiscent of a leucine zipper .
	manualset3
153857	6	408340	13	NULL	NULL	0	NULL	leucine zipper	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The N-terminal region in rat TBP1 , TBP7 , and SUG1 contains a heptad repeat of hydrophobic amino acids reminiscent of a leucine zipper .
	manualset3
153897	1	408341	13	NULL	NULL	0	NULL	N ( 0 ) - P complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The N ( 0 ) - P complex presumably mediates specific encapsidation of the viral genome RNA .
	manualset3
153898	2	408341	13	NULL	NULL	0	NULL	encapsidation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The N ( 0 ) - P complex presumably mediates specific encapsidation of the viral genome RNA .
	manualset3
153899	3	408341	13	NULL	NULL	0	NULL	viral genome RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The N ( 0 ) - P complex presumably mediates specific encapsidation of the viral genome RNA .
	manualset3
153905	1	408342	13	NULL	NULL	0	NULL	N1 feeding interneurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The N1 or N2 feeding interneurons in the buccal ganglia were filled with the fluorescent dye 5 ( 6 ) - carboxyfluorescein ( 5-CF ) from the cut end of the nerve that contains their axon .
	manualset3
153906	2	408342	13	NULL	NULL	0	NULL	N2 feeding interneurons 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The N1 or N2 feeding interneurons in the buccal ganglia were filled with the fluorescent dye 5 ( 6 ) - carboxyfluorescein ( 5-CF ) from the cut end of the nerve that contains their axon .
	manualset3
153907	3	408342	13	NULL	NULL	0	NULL	buccal ganglia	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The N1 or N2 feeding interneurons in the buccal ganglia were filled with the fluorescent dye 5 ( 6 ) - carboxyfluorescein ( 5-CF ) from the cut end of the nerve that contains their axon .
	manualset3
153908	4	408342	13	NULL	NULL	0	NULL	fluorescent dye 5 ( 6 ) - carboxyfluorescein ( 5-CF )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The N1 or N2 feeding interneurons in the buccal ganglia were filled with the fluorescent dye 5 ( 6 ) - carboxyfluorescein ( 5-CF ) from the cut end of the nerve that contains their axon .
	manualset3
153910	5	408342	13	NULL	NULL	0	NULL	 cut end of the nerve	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The N1 or N2 feeding interneurons in the buccal ganglia were filled with the fluorescent dye 5 ( 6 ) - carboxyfluorescein ( 5-CF ) from the cut end of the nerve that contains their axon .
	manualset3
153911	6	408342	13	NULL	NULL	0	NULL	axon 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The N1 or N2 feeding interneurons in the buccal ganglia were filled with the fluorescent dye 5 ( 6 ) - carboxyfluorescein ( 5-CF ) from the cut end of the nerve that contains their axon .
	manualset3
153913	1	408343	13	NULL	NULL	0	NULL	NA-ACCORD ( North American AIDS Cohort Collaboration on Research and Design ) study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The NA-ACCORD ( North American AIDS Cohort Collaboration on Research and Design ) study compared long-term outcomes of immediate versus deferred therapy at 2 CD4 + cell count thresholds .
	manualset3
153914	2	408343	13	NULL	NULL	0	NULL	outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The NA-ACCORD ( North American AIDS Cohort Collaboration on Research and Design ) study compared long-term outcomes of immediate versus deferred therapy at 2 CD4 + cell count thresholds .
	manualset3
153915	3	408343	13	NULL	NULL	NULL	NULL	therapy 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The NA-ACCORD ( North American AIDS Cohort Collaboration on Research and Design ) study compared long-term outcomes of immediate versus deferred therapy at 2 CD4 + cell count thresholds .
	manualset3
153921	4	408343	13	NULL	NULL	0	NULL	2 CD4 + cell count thresholds	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The NA-ACCORD ( North American AIDS Cohort Collaboration on Research and Design ) study compared long-term outcomes of immediate versus deferred therapy at 2 CD4 + cell count thresholds .
	manualset3
153925	1	408344	13	NULL	NULL	0	NULL	 NF-B DNA binding activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The NF-B DNA binding activity of four of those SLs as well as from compounds representing structural parts of the SLs is reported in this article .
	manualset3
153926	2	408344	13	NULL	NULL	0	NULL	four 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The NF-B DNA binding activity of four of those SLs as well as from compounds representing structural parts of the SLs is reported in this article .
	manualset3
153927	3	408344	13	NULL	NULL	0	NULL	SLs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The NF-B DNA binding activity of four of those SLs as well as from compounds representing structural parts of the SLs is reported in this article .
	manualset3
153928	4	408344	13	NULL	NULL	0	NULL	compounds 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The NF-B DNA binding activity of four of those SLs as well as from compounds representing structural parts of the SLs is reported in this article .
	manualset3
153929	5	408344	13	NULL	NULL	0	NULL	structural parts	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The NF-B DNA binding activity of four of those SLs as well as from compounds representing structural parts of the SLs is reported in this article .
	manualset3
153930	6	408344	13	NULL	NULL	0	NULL	SLs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The NF-B DNA binding activity of four of those SLs as well as from compounds representing structural parts of the SLs is reported in this article .
	manualset3
153931	7	408344	13	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The NF-B DNA binding activity of four of those SLs as well as from compounds representing structural parts of the SLs is reported in this article .
	manualset3
153932	1	408345	13	NULL	NULL	0	NULL	NF2 protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The NF2 protein , merlin or schwannomin belongs to the Ezrin , Radixin , Moesin ( ERM ) family involved in the cytoskeletal network and has a tumor suppressor function .
	manualset3
153933	2	408345	13	NULL	NULL	0	NULL	merlin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The NF2 protein , merlin or schwannomin belongs to the Ezrin , Radixin , Moesin ( ERM ) family involved in the cytoskeletal network and has a tumor suppressor function .
	manualset3
153934	3	408345	13	NULL	NULL	0	NULL	schwannomin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The NF2 protein , merlin or schwannomin belongs to the Ezrin , Radixin , Moesin ( ERM ) family involved in the cytoskeletal network and has a tumor suppressor function .
	manualset3
153935	4	408345	13	NULL	NULL	0	NULL	Ezrin , Radixin , Moesin ( ERM ) family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The NF2 protein , merlin or schwannomin belongs to the Ezrin , Radixin , Moesin ( ERM ) family involved in the cytoskeletal network and has a tumor suppressor function .
	manualset3
153938	5	408345	13	NULL	NULL	0	NULL	cytoskeletal network 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The NF2 protein , merlin or schwannomin belongs to the Ezrin , Radixin , Moesin ( ERM ) family involved in the cytoskeletal network and has a tumor suppressor function .
	manualset3
153939	6	408345	13	NULL	NULL	0	NULL	 tumor suppressor function 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The NF2 protein , merlin or schwannomin belongs to the Ezrin , Radixin , Moesin ( ERM ) family involved in the cytoskeletal network and has a tumor suppressor function .
	manualset3
153940	1	408346	13	NULL	NULL	0	NULL	NFKB2 ( lyt-10 ) gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The NFKB2 ( lyt-10 ) gene codes for a protein that is a member of the NK-kappa B/rel family of transcription factors containing a DNA-binding rel domain and a carboxy-terminal ankyrin-like domain .
	manualset3
153942	3	408346	13	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The NFKB2 ( lyt-10 ) gene codes for a protein that is a member of the NK-kappa B/rel family of transcription factors containing a DNA-binding rel domain and a carboxy-terminal ankyrin-like domain .
	manualset3
153943	4	408346	13	NULL	NULL	0	NULL	member	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The NFKB2 ( lyt-10 ) gene codes for a protein that is a member of the NK-kappa B/rel family of transcription factors containing a DNA-binding rel domain and a carboxy-terminal ankyrin-like domain .
	manualset3
153945	5	408346	13	NULL	NULL	0	NULL	NK-kappa B/rel family of transcription factors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The NFKB2 ( lyt-10 ) gene codes for a protein that is a member of the NK-kappa B/rel family of transcription factors containing a DNA-binding rel domain and a carboxy-terminal ankyrin-like domain .
	manualset3
153946	6	408346	13	NULL	NULL	0	NULL	 DNA-binding rel domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The NFKB2 ( lyt-10 ) gene codes for a protein that is a member of the NK-kappa B/rel family of transcription factors containing a DNA-binding rel domain and a carboxy-terminal ankyrin-like domain .
	manualset3
153947	7	408346	13	NULL	NULL	0	NULL	carboxy-terminal ankyrin-like domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The NFKB2 ( lyt-10 ) gene codes for a protein that is a member of the NK-kappa B/rel family of transcription factors containing a DNA-binding rel domain and a carboxy-terminal ankyrin-like domain .
	manualset3
153948	1	408347	13	NULL	NULL	0	NULL	NH -- FC dipole orientation effect	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The NH -- FC dipole orientation effect for pendant exocyclic CH ( 2 ) F .
	manualset3
153949	2	408347	13	NULL	NULL	0	NULL	pendant exocyclic CH ( 2 ) F	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The NH -- FC dipole orientation effect for pendant exocyclic CH ( 2 ) F .
	manualset3
153961	1	408348	13	NULL	NULL	0	NULL	NH	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The NH showed significantly higher flow rates at low lung volumes , that is , FEF75 and FEF75-85 % ( FEF75 : 2.03 ( 0.69 ) vs. 1.70 ( 0.52 ) L/s , p = 0.0092 ; FEF75-85 % : 1.42 ( 0.54 ) vs. 1.06 ( 0.35 ) L/s , p = 0.0001 ) .
	manualset3
153962	2	408348	13	NULL	NULL	0	NULL	flow rates	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The NH showed significantly higher flow rates at low lung volumes , that is , FEF75 and FEF75-85 % ( FEF75 : 2.03 ( 0.69 ) vs. 1.70 ( 0.52 ) L/s , p = 0.0092 ; FEF75-85 % : 1.42 ( 0.54 ) vs. 1.06 ( 0.35 ) L/s , p = 0.0001 ) .
	manualset3
153963	3	408348	13	NULL	NULL	0	NULL	lung volumes	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The NH showed significantly higher flow rates at low lung volumes , that is , FEF75 and FEF75-85 % ( FEF75 : 2.03 ( 0.69 ) vs. 1.70 ( 0.52 ) L/s , p = 0.0092 ; FEF75-85 % : 1.42 ( 0.54 ) vs. 1.06 ( 0.35 ) L/s , p = 0.0001 ) .
	manualset3
153974	4	408348	13	NULL	NULL	0	NULL	FEF75	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The NH showed significantly higher flow rates at low lung volumes , that is , FEF75 and FEF75-85 % ( FEF75 : 2.03 ( 0.69 ) vs. 1.70 ( 0.52 ) L/s , p = 0.0092 ; FEF75-85 % : 1.42 ( 0.54 ) vs. 1.06 ( 0.35 ) L/s , p = 0.0001 ) .
	manualset3
153975	5	408348	13	NULL	NULL	0	NULL	FEF75-85 %	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The NH showed significantly higher flow rates at low lung volumes , that is , FEF75 and FEF75-85 % ( FEF75 : 2.03 ( 0.69 ) vs. 1.70 ( 0.52 ) L/s , p = 0.0092 ; FEF75-85 % : 1.42 ( 0.54 ) vs. 1.06 ( 0.35 ) L/s , p = 0.0001 ) .
	manualset3
153976	6	408348	13	NULL	NULL	NULL	NULL	FEF75 : 2.03 ( 0.69 ) vs. 1.70 ( 0.52 ) L/s 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The NH showed significantly higher flow rates at low lung volumes , that is , FEF75 and FEF75-85 % ( FEF75 : 2.03 ( 0.69 ) vs. 1.70 ( 0.52 ) L/s , p = 0.0092 ; FEF75-85 % : 1.42 ( 0.54 ) vs. 1.06 ( 0.35 ) L/s , p = 0.0001 ) .
	manualset3
153977	7	408348	13	NULL	NULL	0	NULL	p = 0.0092	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The NH showed significantly higher flow rates at low lung volumes , that is , FEF75 and FEF75-85 % ( FEF75 : 2.03 ( 0.69 ) vs. 1.70 ( 0.52 ) L/s , p = 0.0092 ; FEF75-85 % : 1.42 ( 0.54 ) vs. 1.06 ( 0.35 ) L/s , p = 0.0001 ) .
	manualset3
153978	8	408348	13	NULL	NULL	NULL	NULL	 FEF75-85 % : 1.42 ( 0.54 ) vs. 1.06 ( 0.35 ) L/s	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The NH showed significantly higher flow rates at low lung volumes , that is , FEF75 and FEF75-85 % ( FEF75 : 2.03 ( 0.69 ) vs. 1.70 ( 0.52 ) L/s , p = 0.0092 ; FEF75-85 % : 1.42 ( 0.54 ) vs. 1.06 ( 0.35 ) L/s , p = 0.0001 ) .
	manualset3
153979	9	408348	13	NULL	NULL	0	NULL	p = 0.0001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The NH showed significantly higher flow rates at low lung volumes , that is , FEF75 and FEF75-85 % ( FEF75 : 2.03 ( 0.69 ) vs. 1.70 ( 0.52 ) L/s , p = 0.0092 ; FEF75-85 % : 1.42 ( 0.54 ) vs. 1.06 ( 0.35 ) L/s , p = 0.0001 ) .
	manualset3
153980	1	408349	13	NULL	NULL	0	NULL	NIH shuffle	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The NIH shuffle , NCATS , and neurology .
	manualset3
153981	2	408349	13	NULL	NULL	0	NULL	NCATS	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The NIH shuffle , NCATS , and neurology .
	manualset3
153982	3	408349	13	NULL	NULL	0	NULL	neurology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The NIH shuffle , NCATS , and neurology .
	manualset3
153995	1	408350	13	NULL	NULL	0	NULL	NOESY spectrum	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The NOESY spectrum confirmed the selective penetration of the aromatic ring of RAH into the - CD cavity in comparison to that of the piperidine ring .
	manualset3
153996	2	408350	13	NULL	NULL	0	NULL	 penetration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The NOESY spectrum confirmed the selective penetration of the aromatic ring of RAH into the - CD cavity in comparison to that of the piperidine ring .
	manualset3
153997	3	408350	13	NULL	NULL	0	NULL	 aromatic ring of RAH	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The NOESY spectrum confirmed the selective penetration of the aromatic ring of RAH into the - CD cavity in comparison to that of the piperidine ring .
	manualset3
153998	4	408350	13	NULL	NULL	0	NULL	CD cavity	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The NOESY spectrum confirmed the selective penetration of the aromatic ring of RAH into the - CD cavity in comparison to that of the piperidine ring .
	manualset3
153999	5	408350	13	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The NOESY spectrum confirmed the selective penetration of the aromatic ring of RAH into the - CD cavity in comparison to that of the piperidine ring .
	manualset3
154000	6	408350	13	NULL	NULL	0	NULL	piperidine ring	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The NOESY spectrum confirmed the selective penetration of the aromatic ring of RAH into the - CD cavity in comparison to that of the piperidine ring .
	manualset3
154001	1	408351	13	NULL	NULL	0	NULL	NOX2 complex 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The NOX2 complex independent anti-inflammatory effect of SOD3 was further characterized in peritonitis , and SOD3 was found to reduce macrophage infiltration independently of NOX2 complex functionality .
	manualset3
154002	2	408351	13	NULL	NULL	0	NULL	anti-inflammatory effect 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The NOX2 complex independent anti-inflammatory effect of SOD3 was further characterized in peritonitis , and SOD3 was found to reduce macrophage infiltration independently of NOX2 complex functionality .
	manualset3
154003	3	408351	13	NULL	NULL	0	NULL	SOD3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The NOX2 complex independent anti-inflammatory effect of SOD3 was further characterized in peritonitis , and SOD3 was found to reduce macrophage infiltration independently of NOX2 complex functionality .
	manualset3
154004	4	408351	13	NULL	NULL	0	NULL	peritonitis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The NOX2 complex independent anti-inflammatory effect of SOD3 was further characterized in peritonitis , and SOD3 was found to reduce macrophage infiltration independently of NOX2 complex functionality .
	manualset3
154005	5	408351	13	NULL	NULL	0	NULL	SOD3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The NOX2 complex independent anti-inflammatory effect of SOD3 was further characterized in peritonitis , and SOD3 was found to reduce macrophage infiltration independently of NOX2 complex functionality .
	manualset3
154006	6	408351	13	NULL	NULL	0	NULL	macrophage infiltration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The NOX2 complex independent anti-inflammatory effect of SOD3 was further characterized in peritonitis , and SOD3 was found to reduce macrophage infiltration independently of NOX2 complex functionality .
	manualset3
154007	7	408351	13	NULL	NULL	0	NULL	NOX2 complex 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The NOX2 complex independent anti-inflammatory effect of SOD3 was further characterized in peritonitis , and SOD3 was found to reduce macrophage infiltration independently of NOX2 complex functionality .
	manualset3
154008	8	408351	13	NULL	NULL	0	NULL	functionality	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The NOX2 complex independent anti-inflammatory effect of SOD3 was further characterized in peritonitis , and SOD3 was found to reduce macrophage infiltration independently of NOX2 complex functionality .
	manualset3
154009	1	408352	13	NULL	NULL	0	NULL	NP microbiota	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The NP microbiota of young children is highly diverse and appears different between seasons .
	manualset3
154010	2	408352	13	NULL	NULL	0	NULL	young children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The NP microbiota of young children is highly diverse and appears different between seasons .
	manualset3
154036	3	408352	13	NULL	NULL	0	NULL	seasons	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The NP microbiota of young children is highly diverse and appears different between seasons .
	manualset3
154043	1	408353	13	NULL	NULL	0	NULL	NRR 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The NRR has since been offering comprehensive information on nuclear receptor structure and function , as well as general facts of interest to the scientific community on meetings , funding and employment opportunities .
	manualset3
154044	2	408353	13	NULL	NULL	0	NULL	 information	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The NRR has since been offering comprehensive information on nuclear receptor structure and function , as well as general facts of interest to the scientific community on meetings , funding and employment opportunities .
	manualset3
154045	3	408353	13	NULL	NULL	0	NULL	nuclear receptor structure	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The NRR has since been offering comprehensive information on nuclear receptor structure and function , as well as general facts of interest to the scientific community on meetings , funding and employment opportunities .
	manualset3
154046	4	408353	13	NULL	NULL	0	NULL	function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The NRR has since been offering comprehensive information on nuclear receptor structure and function , as well as general facts of interest to the scientific community on meetings , funding and employment opportunities .
	manualset3
154047	5	408353	13	NULL	NULL	NULL	NULL	general facts 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The NRR has since been offering comprehensive information on nuclear receptor structure and function , as well as general facts of interest to the scientific community on meetings , funding and employment opportunities .
	manualset3
154048	6	408353	13	NULL	NULL	0	NULL	interest	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The NRR has since been offering comprehensive information on nuclear receptor structure and function , as well as general facts of interest to the scientific community on meetings , funding and employment opportunities .
	manualset3
154049	7	408353	13	NULL	NULL	0	NULL	scientific community	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The NRR has since been offering comprehensive information on nuclear receptor structure and function , as well as general facts of interest to the scientific community on meetings , funding and employment opportunities .
	manualset3
154050	8	408353	13	NULL	NULL	0	NULL	 meetings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The NRR has since been offering comprehensive information on nuclear receptor structure and function , as well as general facts of interest to the scientific community on meetings , funding and employment opportunities .
	manualset3
154051	9	408353	13	NULL	NULL	0	NULL	funding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The NRR has since been offering comprehensive information on nuclear receptor structure and function , as well as general facts of interest to the scientific community on meetings , funding and employment opportunities .
	manualset3
154052	10	408353	13	NULL	NULL	0	NULL	employment opportunities 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The NRR has since been offering comprehensive information on nuclear receptor structure and function , as well as general facts of interest to the scientific community on meetings , funding and employment opportunities .
	manualset3
154053	1	408354	13	NULL	NULL	0	NULL	Na + channel 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The Na + channel is permeable to Li + and is somewhat permeable to formamidinium , guanidinium and ammonium ions .
	manualset3
154054	2	408354	13	NULL	NULL	0	NULL	 Li +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The Na + channel is permeable to Li + and is somewhat permeable to formamidinium , guanidinium and ammonium ions .
	manualset3
154055	3	408354	13	NULL	NULL	0	NULL	formamidinium ion	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The Na + channel is permeable to Li + and is somewhat permeable to formamidinium , guanidinium and ammonium ions .
	manualset3
154056	4	408354	13	NULL	NULL	0	NULL	guanidinium ion	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The Na + channel is permeable to Li + and is somewhat permeable to formamidinium , guanidinium and ammonium ions .
	manualset3
154057	5	408354	13	NULL	NULL	0	NULL	ammonium ion	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The Na + channel is permeable to Li + and is somewhat permeable to formamidinium , guanidinium and ammonium ions .
	manualset3
154058	1	408355	13	NULL	NULL	0	NULL	Na : K ratios	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Na : K ratios of 9 dogs were & lt ; 20 , being with the most prevalent with the disease of renal failures ( 55.6 % ) .
	manualset3
154059	2	408355	13	NULL	NULL	0	NULL	9 dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The Na : K ratios of 9 dogs were & lt ; 20 , being with the most prevalent with the disease of renal failures ( 55.6 % ) .
	manualset3
154060	3	408355	13	NULL	NULL	0	NULL	 20 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Na : K ratios of 9 dogs were & lt ; 20 , being with the most prevalent with the disease of renal failures ( 55.6 % ) .
	manualset3
154061	4	408355	13	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The Na : K ratios of 9 dogs were & lt ; 20 , being with the most prevalent with the disease of renal failures ( 55.6 % ) .
	manualset3
154062	5	408355	13	NULL	NULL	0	NULL	renal failures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Na : K ratios of 9 dogs were & lt ; 20 , being with the most prevalent with the disease of renal failures ( 55.6 % ) .
	manualset3
154063	6	408355	13	NULL	NULL	0	NULL	 55.6 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Na : K ratios of 9 dogs were & lt ; 20 , being with the most prevalent with the disease of renal failures ( 55.6 % ) .
	manualset3
154064	1	408356	13	NULL	NULL	0	NULL	National Database of Nursing Quality Indicators ( NDNQI )	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The National Database of Nursing Quality Indicators ( NDNQI ) Pressure Ulcer Training Program was developed to improve nursing accuracy and reliability in identifying and staging pressure ulcers and differentiating hospital - and unit-acquired from community-acquired pressure ulcers .
	manualset3
154065	2	408356	13	NULL	NULL	0	NULL	Pressure Ulcer Training Program	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The National Database of Nursing Quality Indicators ( NDNQI ) Pressure Ulcer Training Program was developed to improve nursing accuracy and reliability in identifying and staging pressure ulcers and differentiating hospital - and unit-acquired from community-acquired pressure ulcers .
	manualset3
154066	3	408356	13	NULL	NULL	0	NULL	accuracy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The National Database of Nursing Quality Indicators ( NDNQI ) Pressure Ulcer Training Program was developed to improve nursing accuracy and reliability in identifying and staging pressure ulcers and differentiating hospital - and unit-acquired from community-acquired pressure ulcers .
	manualset3
154067	4	408356	13	NULL	NULL	0	NULL	 reliability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The National Database of Nursing Quality Indicators ( NDNQI ) Pressure Ulcer Training Program was developed to improve nursing accuracy and reliability in identifying and staging pressure ulcers and differentiating hospital - and unit-acquired from community-acquired pressure ulcers .
	manualset3
154068	5	408356	13	NULL	NULL	0	NULL	pressure ulcers 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The National Database of Nursing Quality Indicators ( NDNQI ) Pressure Ulcer Training Program was developed to improve nursing accuracy and reliability in identifying and staging pressure ulcers and differentiating hospital - and unit-acquired from community-acquired pressure ulcers .
	manualset3
154069	6	408356	13	NULL	NULL	0	NULL	hospital-acquired pressure ulcers	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The National Database of Nursing Quality Indicators ( NDNQI ) Pressure Ulcer Training Program was developed to improve nursing accuracy and reliability in identifying and staging pressure ulcers and differentiating hospital - and unit-acquired from community-acquired pressure ulcers .
	manualset3
154070	7	408356	13	NULL	NULL	0	NULL	unit-acquired  pressure ulcers	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The National Database of Nursing Quality Indicators ( NDNQI ) Pressure Ulcer Training Program was developed to improve nursing accuracy and reliability in identifying and staging pressure ulcers and differentiating hospital - and unit-acquired from community-acquired pressure ulcers .
	manualset3
154071	7	408356	13	NULL	NULL	NULL	NULL	community-acquired pressure ulcers	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The National Database of Nursing Quality Indicators ( NDNQI ) Pressure Ulcer Training Program was developed to improve nursing accuracy and reliability in identifying and staging pressure ulcers and differentiating hospital - and unit-acquired from community-acquired pressure ulcers .
	manualset3
154085	1	408357	13	NULL	NULL	0	NULL	reflection model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A reflection model is presented in order to analyze the degree of integration in collaborative work and may serve as an analytical tool for addressing the linkage between different levels of collaboration and identifying opportunities and limitations .
	manualset3
154086	2	408357	13	NULL	NULL	0	NULL	order	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A reflection model is presented in order to analyze the degree of integration in collaborative work and may serve as an analytical tool for addressing the linkage between different levels of collaboration and identifying opportunities and limitations .
	manualset3
154087	3	408357	13	NULL	NULL	0	NULL	degree of integration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A reflection model is presented in order to analyze the degree of integration in collaborative work and may serve as an analytical tool for addressing the linkage between different levels of collaboration and identifying opportunities and limitations .
	manualset3
154088	4	408357	13	NULL	NULL	0	NULL	collaborative work	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A reflection model is presented in order to analyze the degree of integration in collaborative work and may serve as an analytical tool for addressing the linkage between different levels of collaboration and identifying opportunities and limitations .
	manualset3
154089	5	408357	13	NULL	NULL	0	NULL	analytical tool	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A reflection model is presented in order to analyze the degree of integration in collaborative work and may serve as an analytical tool for addressing the linkage between different levels of collaboration and identifying opportunities and limitations .
	manualset3
154090	6	408357	13	NULL	NULL	NULL	NULL	linkage	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A reflection model is presented in order to analyze the degree of integration in collaborative work and may serve as an analytical tool for addressing the linkage between different levels of collaboration and identifying opportunities and limitations .
	manualset3
154091	7	408357	13	NULL	NULL	0	NULL	levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A reflection model is presented in order to analyze the degree of integration in collaborative work and may serve as an analytical tool for addressing the linkage between different levels of collaboration and identifying opportunities and limitations .
	manualset3
154092	8	408357	13	NULL	NULL	0	NULL	collaboration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A reflection model is presented in order to analyze the degree of integration in collaborative work and may serve as an analytical tool for addressing the linkage between different levels of collaboration and identifying opportunities and limitations .
	manualset3
154093	9	408357	13	NULL	NULL	0	NULL	opportunities 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A reflection model is presented in order to analyze the degree of integration in collaborative work and may serve as an analytical tool for addressing the linkage between different levels of collaboration and identifying opportunities and limitations .
	manualset3
154096	10	408357	13	NULL	NULL	0	NULL	limitations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A reflection model is presented in order to analyze the degree of integration in collaborative work and may serve as an analytical tool for addressing the linkage between different levels of collaboration and identifying opportunities and limitations .
	manualset3
154102	1	408358	13	NULL	NULL	0	NULL	 Notch ligand Serrate1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The Notch ligand Serrate1 , expressed in supporting cells in the ear , is regulated by lateral induction , not lateral inhibition ; commitment to become a hair cell is not simply controlled by levels of expression of the Notch ligands Delta1 , Serrate1 , and Serrate2 in the neighbors of the nascent hair cell ; and at least one factor , Numb , capable of blocking reception of lateral inhibition is concentrated in hair cells .
	manualset3
154103	2	408358	13	NULL	NULL	0	NULL	cells	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The Notch ligand Serrate1 , expressed in supporting cells in the ear , is regulated by lateral induction , not lateral inhibition ; commitment to become a hair cell is not simply controlled by levels of expression of the Notch ligands Delta1 , Serrate1 , and Serrate2 in the neighbors of the nascent hair cell ; and at least one factor , Numb , capable of blocking reception of lateral inhibition is concentrated in hair cells .
	manualset3
154104	3	408358	13	NULL	NULL	0	NULL	ear	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The Notch ligand Serrate1 , expressed in supporting cells in the ear , is regulated by lateral induction , not lateral inhibition ; commitment to become a hair cell is not simply controlled by levels of expression of the Notch ligands Delta1 , Serrate1 , and Serrate2 in the neighbors of the nascent hair cell ; and at least one factor , Numb , capable of blocking reception of lateral inhibition is concentrated in hair cells .
	manualset3
154105	4	408358	13	NULL	NULL	0	NULL	lateral induction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Notch ligand Serrate1 , expressed in supporting cells in the ear , is regulated by lateral induction , not lateral inhibition ; commitment to become a hair cell is not simply controlled by levels of expression of the Notch ligands Delta1 , Serrate1 , and Serrate2 in the neighbors of the nascent hair cell ; and at least one factor , Numb , capable of blocking reception of lateral inhibition is concentrated in hair cells .
	manualset3
154106	5	408358	13	NULL	NULL	0	NULL	 lateral inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Notch ligand Serrate1 , expressed in supporting cells in the ear , is regulated by lateral induction , not lateral inhibition ; commitment to become a hair cell is not simply controlled by levels of expression of the Notch ligands Delta1 , Serrate1 , and Serrate2 in the neighbors of the nascent hair cell ; and at least one factor , Numb , capable of blocking reception of lateral inhibition is concentrated in hair cells .
	manualset3
154107	6	408358	13	NULL	NULL	0	NULL	commitment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Notch ligand Serrate1 , expressed in supporting cells in the ear , is regulated by lateral induction , not lateral inhibition ; commitment to become a hair cell is not simply controlled by levels of expression of the Notch ligands Delta1 , Serrate1 , and Serrate2 in the neighbors of the nascent hair cell ; and at least one factor , Numb , capable of blocking reception of lateral inhibition is concentrated in hair cells .
	manualset3
154108	7	408358	13	NULL	NULL	0	NULL	hair cell	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The Notch ligand Serrate1 , expressed in supporting cells in the ear , is regulated by lateral induction , not lateral inhibition ; commitment to become a hair cell is not simply controlled by levels of expression of the Notch ligands Delta1 , Serrate1 , and Serrate2 in the neighbors of the nascent hair cell ; and at least one factor , Numb , capable of blocking reception of lateral inhibition is concentrated in hair cells .
	manualset3
154109	8	408358	13	NULL	NULL	0	NULL	levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Notch ligand Serrate1 , expressed in supporting cells in the ear , is regulated by lateral induction , not lateral inhibition ; commitment to become a hair cell is not simply controlled by levels of expression of the Notch ligands Delta1 , Serrate1 , and Serrate2 in the neighbors of the nascent hair cell ; and at least one factor , Numb , capable of blocking reception of lateral inhibition is concentrated in hair cells .
	manualset3
154110	9	408358	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Notch ligand Serrate1 , expressed in supporting cells in the ear , is regulated by lateral induction , not lateral inhibition ; commitment to become a hair cell is not simply controlled by levels of expression of the Notch ligands Delta1 , Serrate1 , and Serrate2 in the neighbors of the nascent hair cell ; and at least one factor , Numb , capable of blocking reception of lateral inhibition is concentrated in hair cells .
	manualset3
154111	10	408358	13	NULL	NULL	0	NULL	Notch ligands Delta1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The Notch ligand Serrate1 , expressed in supporting cells in the ear , is regulated by lateral induction , not lateral inhibition ; commitment to become a hair cell is not simply controlled by levels of expression of the Notch ligands Delta1 , Serrate1 , and Serrate2 in the neighbors of the nascent hair cell ; and at least one factor , Numb , capable of blocking reception of lateral inhibition is concentrated in hair cells .
	manualset3
154112	11	408358	13	NULL	NULL	0	NULL	Serrate1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The Notch ligand Serrate1 , expressed in supporting cells in the ear , is regulated by lateral induction , not lateral inhibition ; commitment to become a hair cell is not simply controlled by levels of expression of the Notch ligands Delta1 , Serrate1 , and Serrate2 in the neighbors of the nascent hair cell ; and at least one factor , Numb , capable of blocking reception of lateral inhibition is concentrated in hair cells .
	manualset3
154113	12	408358	13	NULL	NULL	0	NULL	Serrate2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The Notch ligand Serrate1 , expressed in supporting cells in the ear , is regulated by lateral induction , not lateral inhibition ; commitment to become a hair cell is not simply controlled by levels of expression of the Notch ligands Delta1 , Serrate1 , and Serrate2 in the neighbors of the nascent hair cell ; and at least one factor , Numb , capable of blocking reception of lateral inhibition is concentrated in hair cells .
	manualset3
154114	13	408358	13	NULL	NULL	0	NULL	neighbors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Notch ligand Serrate1 , expressed in supporting cells in the ear , is regulated by lateral induction , not lateral inhibition ; commitment to become a hair cell is not simply controlled by levels of expression of the Notch ligands Delta1 , Serrate1 , and Serrate2 in the neighbors of the nascent hair cell ; and at least one factor , Numb , capable of blocking reception of lateral inhibition is concentrated in hair cells .
	manualset3
154115	14	408358	13	NULL	NULL	0	NULL	nascent hair cell	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The Notch ligand Serrate1 , expressed in supporting cells in the ear , is regulated by lateral induction , not lateral inhibition ; commitment to become a hair cell is not simply controlled by levels of expression of the Notch ligands Delta1 , Serrate1 , and Serrate2 in the neighbors of the nascent hair cell ; and at least one factor , Numb , capable of blocking reception of lateral inhibition is concentrated in hair cells .
	manualset3
154116	15	408358	13	NULL	NULL	0	NULL	one factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The Notch ligand Serrate1 , expressed in supporting cells in the ear , is regulated by lateral induction , not lateral inhibition ; commitment to become a hair cell is not simply controlled by levels of expression of the Notch ligands Delta1 , Serrate1 , and Serrate2 in the neighbors of the nascent hair cell ; and at least one factor , Numb , capable of blocking reception of lateral inhibition is concentrated in hair cells .
	manualset3
154117	16	408358	13	NULL	NULL	0	NULL	Numb 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The Notch ligand Serrate1 , expressed in supporting cells in the ear , is regulated by lateral induction , not lateral inhibition ; commitment to become a hair cell is not simply controlled by levels of expression of the Notch ligands Delta1 , Serrate1 , and Serrate2 in the neighbors of the nascent hair cell ; and at least one factor , Numb , capable of blocking reception of lateral inhibition is concentrated in hair cells .
	manualset3
154118	17	408358	13	NULL	NULL	0	NULL	reception	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Notch ligand Serrate1 , expressed in supporting cells in the ear , is regulated by lateral induction , not lateral inhibition ; commitment to become a hair cell is not simply controlled by levels of expression of the Notch ligands Delta1 , Serrate1 , and Serrate2 in the neighbors of the nascent hair cell ; and at least one factor , Numb , capable of blocking reception of lateral inhibition is concentrated in hair cells .
	manualset3
154119	18	408358	13	NULL	NULL	0	NULL	lateral inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Notch ligand Serrate1 , expressed in supporting cells in the ear , is regulated by lateral induction , not lateral inhibition ; commitment to become a hair cell is not simply controlled by levels of expression of the Notch ligands Delta1 , Serrate1 , and Serrate2 in the neighbors of the nascent hair cell ; and at least one factor , Numb , capable of blocking reception of lateral inhibition is concentrated in hair cells .
	manualset3
154120	19	408358	13	NULL	NULL	0	NULL	hair cells	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The Notch ligand Serrate1 , expressed in supporting cells in the ear , is regulated by lateral induction , not lateral inhibition ; commitment to become a hair cell is not simply controlled by levels of expression of the Notch ligands Delta1 , Serrate1 , and Serrate2 in the neighbors of the nascent hair cell ; and at least one factor , Numb , capable of blocking reception of lateral inhibition is concentrated in hair cells .
	manualset3
154121	1	408359	13	NULL	NULL	0	NULL	Nubian Complex 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The Nubian Complex of Dhofar , Oman : an African Middle Stone Age industry in Southern Arabia .
	manualset3
154122	2	408359	13	NULL	NULL	0	NULL	Dhofar	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The Nubian Complex of Dhofar , Oman : an African Middle Stone Age industry in Southern Arabia .
	manualset3
154123	3	408359	13	NULL	NULL	0	NULL	Oman	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The Nubian Complex of Dhofar , Oman : an African Middle Stone Age industry in Southern Arabia .
	manualset3
154124	4	408359	13	NULL	NULL	0	NULL	African Middle Stone Age industry 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The Nubian Complex of Dhofar , Oman : an African Middle Stone Age industry in Southern Arabia .
	manualset3
154125	5	408359	13	NULL	NULL	0	NULL	Southern Arabia	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The Nubian Complex of Dhofar , Oman : an African Middle Stone Age industry in Southern Arabia .
	manualset3
154126	1	408360	13	NULL	NULL	0	NULL	O-J-phase	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The O-J-phase in the 0.01-1 ms time range is much less sensitive to light adaptation than the other phases in the 1-200 ms range .
	manualset3
154127	2	408360	13	NULL	NULL	0	NULL	0.01-1 ms time range 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The O-J-phase in the 0.01-1 ms time range is much less sensitive to light adaptation than the other phases in the 1-200 ms range .
	manualset3
154128	3	408360	13	NULL	NULL	0	NULL	adaptation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The O-J-phase in the 0.01-1 ms time range is much less sensitive to light adaptation than the other phases in the 1-200 ms range .
	manualset3
154129	4	408360	13	NULL	NULL	0	NULL	 phases	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The O-J-phase in the 0.01-1 ms time range is much less sensitive to light adaptation than the other phases in the 1-200 ms range .
	manualset3
154130	5	408360	13	NULL	NULL	0	NULL	1-200 ms range 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The O-J-phase in the 0.01-1 ms time range is much less sensitive to light adaptation than the other phases in the 1-200 ms range .
	manualset3
154184	1	408361	13	NULL	NULL	0	NULL	OCAW	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The OCAW , with the Labor Institute , developed a hazardous waste worker and hazardous materials emergency responder health and safety training program that was specific to its members in the represented industries .
	manualset3
154185	2	408361	13	NULL	NULL	0	NULL	Labor Institute	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The OCAW , with the Labor Institute , developed a hazardous waste worker and hazardous materials emergency responder health and safety training program that was specific to its members in the represented industries .
	manualset3
154186	3	408361	13	NULL	NULL	0	NULL	hazardous waste worker	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The OCAW , with the Labor Institute , developed a hazardous waste worker and hazardous materials emergency responder health and safety training program that was specific to its members in the represented industries .
	manualset3
154187	4	408361	13	NULL	NULL	0	NULL	hazardous materials emergency responder health and safety training program	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The OCAW , with the Labor Institute , developed a hazardous waste worker and hazardous materials emergency responder health and safety training program that was specific to its members in the represented industries .
	manualset3
154188	5	408361	13	NULL	NULL	0	NULL	 members	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The OCAW , with the Labor Institute , developed a hazardous waste worker and hazardous materials emergency responder health and safety training program that was specific to its members in the represented industries .
	manualset3
154189	6	408361	13	NULL	NULL	0	NULL	industries	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The OCAW , with the Labor Institute , developed a hazardous waste worker and hazardous materials emergency responder health and safety training program that was specific to its members in the represented industries .
	manualset3
154190	1	408362	13	NULL	NULL	0	NULL	OHS measure	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The OHS measure is introduced by replacing the distance concept of conventional Hausdoff distance ( HD ) algorithms by the similarity concept of the Hough transform ( HT ) .
	manualset3
154191	2	408362	13	NULL	NULL	0	NULL	 distance concept 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The OHS measure is introduced by replacing the distance concept of conventional Hausdoff distance ( HD ) algorithms by the similarity concept of the Hough transform ( HT ) .
	manualset3
154192	3	408362	13	NULL	NULL	0	NULL	conventional Hausdoff distance ( HD ) algorithms 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The OHS measure is introduced by replacing the distance concept of conventional Hausdoff distance ( HD ) algorithms by the similarity concept of the Hough transform ( HT ) .
	manualset3
154193	4	408362	13	NULL	NULL	0	NULL	similarity concept of the Hough transform ( HT ) 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The OHS measure is introduced by replacing the distance concept of conventional Hausdoff distance ( HD ) algorithms by the similarity concept of the Hough transform ( HT ) .
	manualset3
154194	1	408363	13	NULL	NULL	0	NULL	OID group 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The OID group was intermediate , 57 % of cases with OB and 43 % with polyclonal CSF IgG patterns .
	manualset3
154195	2	408363	13	NULL	NULL	0	NULL	 57 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The OID group was intermediate , 57 % of cases with OB and 43 % with polyclonal CSF IgG patterns .
	manualset3
154196	3	408363	13	NULL	NULL	0	NULL	 cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The OID group was intermediate , 57 % of cases with OB and 43 % with polyclonal CSF IgG patterns .
	manualset3
154197	4	408363	13	NULL	NULL	0	NULL	 OB	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The OID group was intermediate , 57 % of cases with OB and 43 % with polyclonal CSF IgG patterns .
	manualset3
154198	5	408363	13	NULL	NULL	0	NULL	43 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The OID group was intermediate , 57 % of cases with OB and 43 % with polyclonal CSF IgG patterns .
	manualset3
154199	6	408363	13	NULL	NULL	0	NULL	polyclonal CSF IgG patterns	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The OID group was intermediate , 57 % of cases with OB and 43 % with polyclonal CSF IgG patterns .
	manualset3
154200	1	408364	13	NULL	NULL	0	NULL	OR	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The OR for mortality was 5.2 ( 95 % CI , 2.5 to 11.2 ; P & lt ; 0.0001 ) in patients with a BD -4 or less .
	manualset3
154201	2	408364	13	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The OR for mortality was 5.2 ( 95 % CI , 2.5 to 11.2 ; P & lt ; 0.0001 ) in patients with a BD -4 or less .
	manualset3
154202	3	408364	13	NULL	NULL	0	NULL	 5.2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The OR for mortality was 5.2 ( 95 % CI , 2.5 to 11.2 ; P & lt ; 0.0001 ) in patients with a BD -4 or less .
	manualset3
154203	4	408364	13	NULL	NULL	NULL	NULL	95 % CI , 2.5 to 11.2	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The OR for mortality was 5.2 ( 95 % CI , 2.5 to 11.2 ; P & lt ; 0.0001 ) in patients with a BD -4 or less .
	manualset3
154204	5	408364	13	NULL	NULL	0	NULL	0.0001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The OR for mortality was 5.2 ( 95 % CI , 2.5 to 11.2 ; P & lt ; 0.0001 ) in patients with a BD -4 or less .
	manualset3
154205	6	408364	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The OR for mortality was 5.2 ( 95 % CI , 2.5 to 11.2 ; P & lt ; 0.0001 ) in patients with a BD -4 or less .
	manualset3
154206	7	408364	13	NULL	NULL	0	NULL	BD -4 or less	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The OR for mortality was 5.2 ( 95 % CI , 2.5 to 11.2 ; P & lt ; 0.0001 ) in patients with a BD -4 or less .
	manualset3
154207	1	408365	13	NULL	NULL	0	NULL	ORS cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The ORS cells , except for the IMCs , seemed to originate mostly from the D-cells .
	manualset3
154208	2	408365	13	NULL	NULL	0	NULL	IMCs 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The ORS cells , except for the IMCs , seemed to originate mostly from the D-cells .
	manualset3
154209	3	408365	13	NULL	NULL	0	NULL	D-cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The ORS cells , except for the IMCs , seemed to originate mostly from the D-cells .
	manualset3
154210	1	408366	13	NULL	NULL	0	NULL	OWFEG free energy grid	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The OWFEG free energy grid is generated from a one-window free energy perturbation MD simulation ( Pearlman , D. A. J. Med .
	manualset3
154211	2	408366	13	NULL	NULL	0	NULL	one-window free energy perturbation MD simulation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The OWFEG free energy grid is generated from a one-window free energy perturbation MD simulation ( Pearlman , D. A. J. Med .
	manualset3
154212	3	408366	13	NULL	NULL	0	NULL	Pearlman	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The OWFEG free energy grid is generated from a one-window free energy perturbation MD simulation ( Pearlman , D. A. J. Med .
	manualset3
154213	4	408366	13	NULL	NULL	0	NULL	D. A. J. Med	Journal												NULL		0	NULL	NULL	NULL	NULL	NULL	The OWFEG free energy grid is generated from a one-window free energy perturbation MD simulation ( Pearlman , D. A. J. Med .
	manualset3
154214	1	408367	13	NULL	NULL	0	NULL	Outside-In model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The Outside-In model has been supported by an autoimmune model for MS , experimental autoimmune ( allergic ) encephalomyelitis ( EAE ) .
	manualset3
154215	2	408367	13	NULL	NULL	0	NULL	autoimmune model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The Outside-In model has been supported by an autoimmune model for MS , experimental autoimmune ( allergic ) encephalomyelitis ( EAE ) .
	manualset3
154216	3	408367	13	NULL	NULL	0	NULL	MS 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The Outside-In model has been supported by an autoimmune model for MS , experimental autoimmune ( allergic ) encephalomyelitis ( EAE ) .
	manualset3
154217	4	408367	13	NULL	NULL	0	NULL	experimental autoimmune ( allergic ) encephalomyelitis ( EAE ) 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The Outside-In model has been supported by an autoimmune model for MS , experimental autoimmune ( allergic ) encephalomyelitis ( EAE ) .
	manualset3
154218	1	408368	13	NULL	NULL	0	NULL	 P-wave	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The P-wave and the PAD produced by mechanical stimulation were at a minimum in the rostral part of the cuneate nucleus and at a maximum 2-6 mm caudal to the obex .3 .
	manualset3
154219	2	408368	13	NULL	NULL	0	NULL	PAD	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The P-wave and the PAD produced by mechanical stimulation were at a minimum in the rostral part of the cuneate nucleus and at a maximum 2-6 mm caudal to the obex .3 .
	manualset3
154220	3	408368	13	NULL	NULL	0	NULL	mechanical stimulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The P-wave and the PAD produced by mechanical stimulation were at a minimum in the rostral part of the cuneate nucleus and at a maximum 2-6 mm caudal to the obex .3 .
	manualset3
154221	4	408368	13	NULL	NULL	0	NULL	minimum	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The P-wave and the PAD produced by mechanical stimulation were at a minimum in the rostral part of the cuneate nucleus and at a maximum 2-6 mm caudal to the obex .3 .
	manualset3
154222	5	408368	13	NULL	NULL	0	NULL	rostral part	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The P-wave and the PAD produced by mechanical stimulation were at a minimum in the rostral part of the cuneate nucleus and at a maximum 2-6 mm caudal to the obex .3 .
	manualset3
154223	6	408368	13	NULL	NULL	0	NULL	cuneate nucleus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The P-wave and the PAD produced by mechanical stimulation were at a minimum in the rostral part of the cuneate nucleus and at a maximum 2-6 mm caudal to the obex .3 .
	manualset3
154224	7	408368	13	NULL	NULL	0	NULL	maximum 2-6 mm 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The P-wave and the PAD produced by mechanical stimulation were at a minimum in the rostral part of the cuneate nucleus and at a maximum 2-6 mm caudal to the obex .3 .
	manualset3
154225	8	408368	13	NULL	NULL	0	NULL	caudal	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The P-wave and the PAD produced by mechanical stimulation were at a minimum in the rostral part of the cuneate nucleus and at a maximum 2-6 mm caudal to the obex .3 .
	manualset3
154226	9	408368	13	NULL	NULL	0	NULL	obex .3	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The P-wave and the PAD produced by mechanical stimulation were at a minimum in the rostral part of the cuneate nucleus and at a maximum 2-6 mm caudal to the obex .3 .
	manualset3
154227	1	408369	13	NULL	NULL	0	NULL	P. multocida GlpQ homolog	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The P. multocida GlpQ homolog showed glycerophosphodiester phosphodiesterase enzyme activity , indicating that it is a functional homolog of other characterized GlpQ enzymes .
	manualset3
154228	2	408369	13	NULL	NULL	0	NULL	glycerophosphodiester phosphodiesterase enzyme activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The P. multocida GlpQ homolog showed glycerophosphodiester phosphodiesterase enzyme activity , indicating that it is a functional homolog of other characterized GlpQ enzymes .
	manualset3
154229	3	408369	13	NULL	NULL	0	NULL	functional homolog	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The P. multocida GlpQ homolog showed glycerophosphodiester phosphodiesterase enzyme activity , indicating that it is a functional homolog of other characterized GlpQ enzymes .
	manualset3
154230	4	408369	13	NULL	NULL	0	NULL	GlpQ enzymes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The P. multocida GlpQ homolog showed glycerophosphodiester phosphodiesterase enzyme activity , indicating that it is a functional homolog of other characterized GlpQ enzymes .
	manualset3
154231	1	408370	13	NULL	NULL	0	NULL	 PAT/DOT system	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The PAT/DOT system offers a spatial resolution of 0.5 mm for PAT and of 4.0 mm for DOT .
	manualset3
154232	2	408370	13	NULL	NULL	0	NULL	spatial resolution	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The PAT/DOT system offers a spatial resolution of 0.5 mm for PAT and of 4.0 mm for DOT .
	manualset3
154233	3	408370	13	NULL	NULL	0	NULL	0.5 mm 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The PAT/DOT system offers a spatial resolution of 0.5 mm for PAT and of 4.0 mm for DOT .
	manualset3
154234	4	408370	13	NULL	NULL	0	NULL	PAT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The PAT/DOT system offers a spatial resolution of 0.5 mm for PAT and of 4.0 mm for DOT .
	manualset3
154235	5	408370	13	NULL	NULL	0	NULL	4.0 mm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The PAT/DOT system offers a spatial resolution of 0.5 mm for PAT and of 4.0 mm for DOT .
	manualset3
154236	6	408370	13	NULL	NULL	0	NULL	DOT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The PAT/DOT system offers a spatial resolution of 0.5 mm for PAT and of 4.0 mm for DOT .
	manualset3
154237	1	408371	13	NULL	NULL	0	NULL	PCNA index	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The PCNA index was closely related to the prognosis of neuroblastoma and to N-myc amplification .
	manualset3
154238	2	408371	13	NULL	NULL	0	NULL	prognosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The PCNA index was closely related to the prognosis of neuroblastoma and to N-myc amplification .
	manualset3
154239	3	408371	13	NULL	NULL	0	NULL	neuroblastoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The PCNA index was closely related to the prognosis of neuroblastoma and to N-myc amplification .
	manualset3
154240	4	408371	13	NULL	NULL	0	NULL	N-myc amplification 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The PCNA index was closely related to the prognosis of neuroblastoma and to N-myc amplification .
	manualset3
154241	1	408372	13	NULL	NULL	0	NULL	PCR test 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The PCR test was positive for CMV DNA .
	manualset3
154242	2	408372	13	NULL	NULL	0	NULL	CMV DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The PCR test was positive for CMV DNA .
	manualset3
154243	1	408373	13	NULL	NULL	0	NULL	Characteristics 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Characteristics of the interpretation and the significance of angiographic findings in recognizing soft tissue tumors of the extremities ) .
	manualset3
154244	2	408373	13	NULL	NULL	0	NULL	 interpretation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Characteristics of the interpretation and the significance of angiographic findings in recognizing soft tissue tumors of the extremities ) .
	manualset3
154245	3	408373	13	NULL	NULL	0	NULL	significance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Characteristics of the interpretation and the significance of angiographic findings in recognizing soft tissue tumors of the extremities ) .
	manualset3
154246	4	408373	13	NULL	NULL	0	NULL	angiographic findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Characteristics of the interpretation and the significance of angiographic findings in recognizing soft tissue tumors of the extremities ) .
	manualset3
154247	5	408373	13	NULL	NULL	0	NULL	soft tissue tumors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Characteristics of the interpretation and the significance of angiographic findings in recognizing soft tissue tumors of the extremities ) .
	manualset3
154248	6	408373	13	NULL	NULL	0	NULL	extremities	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Characteristics of the interpretation and the significance of angiographic findings in recognizing soft tissue tumors of the extremities ) .
	manualset3
154249	1	408374	13	NULL	NULL	0	NULL	regulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A regulation requiring the use of proper prescriptions and detailed records for the supply and dispensing of benzodiazepines , appears to have curbed , at least partially , their abuse in Hong Kong .
	manualset3
154250	2	408374	13	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A regulation requiring the use of proper prescriptions and detailed records for the supply and dispensing of benzodiazepines , appears to have curbed , at least partially , their abuse in Hong Kong .
	manualset3
154251	3	408374	13	NULL	NULL	0	NULL	prescriptions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A regulation requiring the use of proper prescriptions and detailed records for the supply and dispensing of benzodiazepines , appears to have curbed , at least partially , their abuse in Hong Kong .
	manualset3
154252	4	408374	13	NULL	NULL	0	NULL	 records	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A regulation requiring the use of proper prescriptions and detailed records for the supply and dispensing of benzodiazepines , appears to have curbed , at least partially , their abuse in Hong Kong .
	manualset3
154253	5	408374	13	NULL	NULL	0	NULL	supply	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A regulation requiring the use of proper prescriptions and detailed records for the supply and dispensing of benzodiazepines , appears to have curbed , at least partially , their abuse in Hong Kong .
	manualset3
154254	6	408374	13	NULL	NULL	0	NULL	benzodiazepines	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A regulation requiring the use of proper prescriptions and detailed records for the supply and dispensing of benzodiazepines , appears to have curbed , at least partially , their abuse in Hong Kong .
	manualset3
154255	7	408374	13	NULL	NULL	0	NULL	abuse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A regulation requiring the use of proper prescriptions and detailed records for the supply and dispensing of benzodiazepines , appears to have curbed , at least partially , their abuse in Hong Kong .
	manualset3
154256	8	408374	13	NULL	NULL	0	NULL	Hong Kong 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A regulation requiring the use of proper prescriptions and detailed records for the supply and dispensing of benzodiazepines , appears to have curbed , at least partially , their abuse in Hong Kong .
	manualset3
154257	1	408375	13	NULL	NULL	0	NULL	PIP Compass hinge	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The PIP Compass hinge is a useful adjunct to surgical reconstruction of the injured PIP joint .
	manualset3
154258	2	408375	13	NULL	NULL	0	NULL	adjunct	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The PIP Compass hinge is a useful adjunct to surgical reconstruction of the injured PIP joint .
	manualset3
154259	3	408375	13	NULL	NULL	0	NULL	surgical reconstruction 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The PIP Compass hinge is a useful adjunct to surgical reconstruction of the injured PIP joint .
	manualset3
154260	4	408375	13	NULL	NULL	0	NULL	PIP joint	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The PIP Compass hinge is a useful adjunct to surgical reconstruction of the injured PIP joint .
	manualset3
154262	1	408376	13	NULL	NULL	0	NULL	PML risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The PML risk in a pooled clinical trial cohort has been estimated to be 1 person for every 1 , 000 patients treated for an average of 17.9 months , although this figure could change in either direction with more experience with the drug .
	manualset3
154265	2	408376	13	NULL	NULL	0	NULL	clinical trial cohort	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The PML risk in a pooled clinical trial cohort has been estimated to be 1 person for every 1 , 000 patients treated for an average of 17.9 months , although this figure could change in either direction with more experience with the drug .
	manualset3
154267	3	408376	13	NULL	NULL	0	NULL	1 person 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The PML risk in a pooled clinical trial cohort has been estimated to be 1 person for every 1 , 000 patients treated for an average of 17.9 months , although this figure could change in either direction with more experience with the drug .
	manualset3
154268	4	408376	13	NULL	NULL	0	NULL	1 , 000 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The PML risk in a pooled clinical trial cohort has been estimated to be 1 person for every 1 , 000 patients treated for an average of 17.9 months , although this figure could change in either direction with more experience with the drug .
	manualset3
154269	5	408376	13	NULL	NULL	0	NULL	average of 17.9 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The PML risk in a pooled clinical trial cohort has been estimated to be 1 person for every 1 , 000 patients treated for an average of 17.9 months , although this figure could change in either direction with more experience with the drug .
	manualset3
154270	6	408376	13	NULL	NULL	0	NULL	figure	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The PML risk in a pooled clinical trial cohort has been estimated to be 1 person for every 1 , 000 patients treated for an average of 17.9 months , although this figure could change in either direction with more experience with the drug .
	manualset3
154271	7	408376	13	NULL	NULL	0	NULL	direction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The PML risk in a pooled clinical trial cohort has been estimated to be 1 person for every 1 , 000 patients treated for an average of 17.9 months , although this figure could change in either direction with more experience with the drug .
	manualset3
154272	8	408376	13	NULL	NULL	0	NULL	experience 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The PML risk in a pooled clinical trial cohort has been estimated to be 1 person for every 1 , 000 patients treated for an average of 17.9 months , although this figure could change in either direction with more experience with the drug .
	manualset3
154273	9	408376	13	NULL	NULL	0	NULL	drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The PML risk in a pooled clinical trial cohort has been estimated to be 1 person for every 1 , 000 patients treated for an average of 17.9 months , although this figure could change in either direction with more experience with the drug .
	manualset3
154275	1	408377	13	NULL	NULL	0	NULL	PNA/DNA/beads conjugate	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The PNA/DNA/beads conjugate was analyzed by MALDI-TOFMS .
	manualset3
154276	2	408377	13	NULL	NULL	0	NULL	MALDI-TOFMS	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The PNA/DNA/beads conjugate was analyzed by MALDI-TOFMS .
	manualset3
154277	1	408378	13	NULL	NULL	0	NULL	PNN inputs 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The PNN inputs were O2 level in the blood , body weight , electrocardiogram ( ECG ) , hematocrit , S wave , and heart rate of individual birds .
	manualset3
154279	2	408378	13	NULL	NULL	0	NULL	O2 level	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The PNN inputs were O2 level in the blood , body weight , electrocardiogram ( ECG ) , hematocrit , S wave , and heart rate of individual birds .
	manualset3
154281	3	408378	13	NULL	NULL	0	NULL	blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The PNN inputs were O2 level in the blood , body weight , electrocardiogram ( ECG ) , hematocrit , S wave , and heart rate of individual birds .
	manualset3
154282	4	408378	13	NULL	NULL	0	NULL	body weight	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The PNN inputs were O2 level in the blood , body weight , electrocardiogram ( ECG ) , hematocrit , S wave , and heart rate of individual birds .
	manualset3
154284	5	408378	13	NULL	NULL	0	NULL	electrocardiogram ( ECG )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The PNN inputs were O2 level in the blood , body weight , electrocardiogram ( ECG ) , hematocrit , S wave , and heart rate of individual birds .
	manualset3
154285	6	408378	13	NULL	NULL	0	NULL	 hematocrit	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The PNN inputs were O2 level in the blood , body weight , electrocardiogram ( ECG ) , hematocrit , S wave , and heart rate of individual birds .
	manualset3
154286	7	408378	13	NULL	NULL	0	NULL	S wave	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The PNN inputs were O2 level in the blood , body weight , electrocardiogram ( ECG ) , hematocrit , S wave , and heart rate of individual birds .
	manualset3
154288	8	408378	13	NULL	NULL	0	NULL	 heart rate 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The PNN inputs were O2 level in the blood , body weight , electrocardiogram ( ECG ) , hematocrit , S wave , and heart rate of individual birds .
	manualset3
154290	9	408378	13	NULL	NULL	0	NULL	individual birds	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The PNN inputs were O2 level in the blood , body weight , electrocardiogram ( ECG ) , hematocrit , S wave , and heart rate of individual birds .
	manualset3
154292	1	408379	13	NULL	NULL	0	NULL	POEMS syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The POEMS syndrome : report of three cases with radiographic abnormalities .
	manualset3
154293	2	408379	13	NULL	NULL	0	NULL	report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The POEMS syndrome : report of three cases with radiographic abnormalities .
	manualset3
154294	3	408379	13	NULL	NULL	0	NULL	three cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The POEMS syndrome : report of three cases with radiographic abnormalities .
	manualset3
154295	4	408379	13	NULL	NULL	0	NULL	radiographic abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The POEMS syndrome : report of three cases with radiographic abnormalities .
	manualset3
154296	1	408380	13	NULL	NULL	0	NULL	 POZ/BTB protein NAC1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The POZ/BTB protein NAC1 interacts with two different histone deacetylases in neuronal-like cultures .
	manualset3
154297	2	408380	13	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The POZ/BTB protein NAC1 interacts with two different histone deacetylases in neuronal-like cultures .
	manualset3
154298	3	408380	13	NULL	NULL	0	NULL	histone deacetylases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The POZ/BTB protein NAC1 interacts with two different histone deacetylases in neuronal-like cultures .
	manualset3
154299	4	408380	13	NULL	NULL	0	NULL	neuronal-like cultures	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The POZ/BTB protein NAC1 interacts with two different histone deacetylases in neuronal-like cultures .
	manualset3
154300	1	408381	13	NULL	NULL	0	NULL	PPACA 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The PPACA contains a variety of reforms that , if implemented , will significantly impact the field of PM & R .
	manualset3
154301	2	408381	13	NULL	NULL	0	NULL	variety of reforms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The PPACA contains a variety of reforms that , if implemented , will significantly impact the field of PM & R .
	manualset3
154315	3	408381	13	NULL	NULL	0	NULL	 impact 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The PPACA contains a variety of reforms that , if implemented , will significantly impact the field of PM & R .
	manualset3
154316	4	408381	13	NULL	NULL	0	NULL	field of PM & R 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The PPACA contains a variety of reforms that , if implemented , will significantly impact the field of PM & R .
	manualset3
154317	1	408382	13	NULL	NULL	0	NULL	PPARG gene expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The PPARG gene expression in liver in the same chicken subsets was also significantly different .
	manualset3
154318	2	408382	13	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The PPARG gene expression in liver in the same chicken subsets was also significantly different .
	manualset3
154319	3	408382	13	NULL	NULL	0	NULL	chicken subsets 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The PPARG gene expression in liver in the same chicken subsets was also significantly different .
	manualset3
154320	1	408383	13	NULL	NULL	0	NULL	PRL phosphatases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The PRL phosphatases , which constitute a subfamily of the protein tyrosine phosphatases ( PTPs ) , are implicated in oncogenic and metastatic processes .
	manualset3
154321	2	408383	13	NULL	NULL	0	NULL	subfamily of the protein tyrosine phosphatases ( PTPs )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The PRL phosphatases , which constitute a subfamily of the protein tyrosine phosphatases ( PTPs ) , are implicated in oncogenic and metastatic processes .
	manualset3
154322	3	408383	13	NULL	NULL	0	NULL	oncogenic processes 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The PRL phosphatases , which constitute a subfamily of the protein tyrosine phosphatases ( PTPs ) , are implicated in oncogenic and metastatic processes .
	manualset3
154323	4	408383	13	NULL	NULL	0	NULL	metastatic processes 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The PRL phosphatases , which constitute a subfamily of the protein tyrosine phosphatases ( PTPs ) , are implicated in oncogenic and metastatic processes .
	manualset3
154324	1	408384	13	NULL	NULL	0	NULL	PSI	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The PSI to DLMn ( Dorsal Longitudinal Muscle neuron ) connection is dependent on D7 nicotinic acetylcholine receptors ( nAChRs ) .
	manualset3
154325	2	408384	13	NULL	NULL	0	NULL	DLMn	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The PSI to DLMn ( Dorsal Longitudinal Muscle neuron ) connection is dependent on D7 nicotinic acetylcholine receptors ( nAChRs ) .
	manualset3
154326	3	408384	13	NULL	NULL	0	NULL	Dorsal Longitudinal Muscle neuron	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The PSI to DLMn ( Dorsal Longitudinal Muscle neuron ) connection is dependent on D7 nicotinic acetylcholine receptors ( nAChRs ) .
	manualset3
154327	4	408384	13	NULL	NULL	0	NULL	connection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The PSI to DLMn ( Dorsal Longitudinal Muscle neuron ) connection is dependent on D7 nicotinic acetylcholine receptors ( nAChRs ) .
	manualset3
154328	5	408384	13	NULL	NULL	0	NULL	D7 nicotinic acetylcholine receptors ( nAChRs ) 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The PSI to DLMn ( Dorsal Longitudinal Muscle neuron ) connection is dependent on D7 nicotinic acetylcholine receptors ( nAChRs ) .
	manualset3
154329	1	408385	13	NULL	NULL	0	NULL	 regulatory SNP	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A regulatory SNP in AKAP13 is associated with blood pressure in Koreans .
	manualset3
154330	2	408385	13	NULL	NULL	0	NULL	AKAP13	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A regulatory SNP in AKAP13 is associated with blood pressure in Koreans .
	manualset3
154331	3	408385	13	NULL	NULL	0	NULL	blood pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A regulatory SNP in AKAP13 is associated with blood pressure in Koreans .
	manualset3
154332	4	408385	13	NULL	NULL	0	NULL	Koreans	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A regulatory SNP in AKAP13 is associated with blood pressure in Koreans .
	manualset3
154333	1	408386	13	NULL	NULL	0	NULL	PVH incidence 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The PVH incidence was 60 % in those of 23-26 weeks and 38 % in those of 27-28 weeks .
	manualset3
154334	2	408386	13	NULL	NULL	0	NULL	60 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The PVH incidence was 60 % in those of 23-26 weeks and 38 % in those of 27-28 weeks .
	manualset3
154335	3	408386	13	NULL	NULL	0	NULL	23-26 weeks 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The PVH incidence was 60 % in those of 23-26 weeks and 38 % in those of 27-28 weeks .
	manualset3
154336	4	408386	13	NULL	NULL	0	NULL	38 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The PVH incidence was 60 % in those of 23-26 weeks and 38 % in those of 27-28 weeks .
	manualset3
154337	5	408386	13	NULL	NULL	0	NULL	27-28 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The PVH incidence was 60 % in those of 23-26 weeks and 38 % in those of 27-28 weeks .
	manualset3
154338	1	408387	13	NULL	NULL	0	NULL	PWP2 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The PWP2 gene is essential for growth because spores carrying the pwp2 delta 1 : : HIS3 disruption germinate before arresting growth with one or two large buds .
	manualset3
154339	2	408387	13	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The PWP2 gene is essential for growth because spores carrying the pwp2 delta 1 : : HIS3 disruption germinate before arresting growth with one or two large buds .
	manualset3
154340	3	408387	13	NULL	NULL	0	NULL	spores	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The PWP2 gene is essential for growth because spores carrying the pwp2 delta 1 : : HIS3 disruption germinate before arresting growth with one or two large buds .
	manualset3
154341	4	408387	13	NULL	NULL	0	NULL	pwp2 delta 1 : : HIS3 disruption 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The PWP2 gene is essential for growth because spores carrying the pwp2 delta 1 : : HIS3 disruption germinate before arresting growth with one or two large buds .
	manualset3
154342	5	408387	13	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The PWP2 gene is essential for growth because spores carrying the pwp2 delta 1 : : HIS3 disruption germinate before arresting growth with one or two large buds .
	manualset3
154343	6	408387	13	NULL	NULL	0	NULL	one or two large buds 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The PWP2 gene is essential for growth because spores carrying the pwp2 delta 1 : : HIS3 disruption germinate before arresting growth with one or two large buds .
	manualset3
154417	1	408388	13	NULL	NULL	0	NULL	Peutz jeghers syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The Peutz jeghers syndrome is a familial affection with dominant autosomic transmission characterized by a hamartoma digestive polyposis and a cutaneous mucous lentiginosis with periorifice predominance .
	manualset3
154418	2	408388	13	NULL	NULL	0	NULL	familial affection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Peutz jeghers syndrome is a familial affection with dominant autosomic transmission characterized by a hamartoma digestive polyposis and a cutaneous mucous lentiginosis with periorifice predominance .
	manualset3
154419	3	408388	13	NULL	NULL	0	NULL	dominant autosomic transmission 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Peutz jeghers syndrome is a familial affection with dominant autosomic transmission characterized by a hamartoma digestive polyposis and a cutaneous mucous lentiginosis with periorifice predominance .
	manualset3
154420	4	408388	13	NULL	NULL	0	NULL	 hamartoma digestive polyposis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Peutz jeghers syndrome is a familial affection with dominant autosomic transmission characterized by a hamartoma digestive polyposis and a cutaneous mucous lentiginosis with periorifice predominance .
	manualset3
154421	5	408388	13	NULL	NULL	0	NULL	cutaneous mucous lentiginosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Peutz jeghers syndrome is a familial affection with dominant autosomic transmission characterized by a hamartoma digestive polyposis and a cutaneous mucous lentiginosis with periorifice predominance .
	manualset3
154422	6	408388	13	NULL	NULL	0	NULL	periorifice predominance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Peutz jeghers syndrome is a familial affection with dominant autosomic transmission characterized by a hamartoma digestive polyposis and a cutaneous mucous lentiginosis with periorifice predominance .
	manualset3
154423	1	408389	13	NULL	NULL	NULL	NULL	Possum mutation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The Possum mutation enhanced Na ( v ) 1.8 sodium currents and neuronal excitability and heightened sensitivity of mutants to cold stimuli .
	manualset3
154424	2	408389	13	NULL	NULL	0	NULL	Na ( v ) 1.8 sodium currents	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Possum mutation enhanced Na ( v ) 1.8 sodium currents and neuronal excitability and heightened sensitivity of mutants to cold stimuli .
	manualset3
154425	3	408389	13	NULL	NULL	0	NULL	neuronal excitability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Possum mutation enhanced Na ( v ) 1.8 sodium currents and neuronal excitability and heightened sensitivity of mutants to cold stimuli .
	manualset3
154426	4	408389	13	NULL	NULL	0	NULL	sensitivity of mutants	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Possum mutation enhanced Na ( v ) 1.8 sodium currents and neuronal excitability and heightened sensitivity of mutants to cold stimuli .
	manualset3
154427	5	408389	13	NULL	NULL	0	NULL	cold stimuli	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Possum mutation enhanced Na ( v ) 1.8 sodium currents and neuronal excitability and heightened sensitivity of mutants to cold stimuli .
	manualset3
154428	1	408390	13	NULL	NULL	0	NULL	Pregnancy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Pregnancy , Infection , and Nutrition Study collected genital tract specimens and documented cervical change from 807 eligible women between 24 and 29 weeks ' gestation .
	manualset3
154429	2	408390	13	NULL	NULL	0	NULL	Infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Pregnancy , Infection , and Nutrition Study collected genital tract specimens and documented cervical change from 807 eligible women between 24 and 29 weeks ' gestation .
	manualset3
154430	3	408390	13	NULL	NULL	0	NULL	Nutrition Study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Pregnancy , Infection , and Nutrition Study collected genital tract specimens and documented cervical change from 807 eligible women between 24 and 29 weeks ' gestation .
	manualset3
154431	4	408390	13	NULL	NULL	0	NULL	genital tract specimens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The Pregnancy , Infection , and Nutrition Study collected genital tract specimens and documented cervical change from 807 eligible women between 24 and 29 weeks ' gestation .
	manualset3
154432	5	408390	13	NULL	NULL	0	NULL	cervical change	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Pregnancy , Infection , and Nutrition Study collected genital tract specimens and documented cervical change from 807 eligible women between 24 and 29 weeks ' gestation .
	manualset3
154433	6	408390	13	NULL	NULL	0	NULL	807 eligible women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The Pregnancy , Infection , and Nutrition Study collected genital tract specimens and documented cervical change from 807 eligible women between 24 and 29 weeks ' gestation .
	manualset3
154434	7	408390	13	NULL	NULL	0	NULL	24 and 29 weeks ' gestation 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The Pregnancy , Infection , and Nutrition Study collected genital tract specimens and documented cervical change from 807 eligible women between 24 and 29 weeks ' gestation .
	manualset3
154435	1	408391	13	NULL	NULL	0	NULL	President 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The President of the United States of America : a neglected person in our emergency medical system .
	manualset3
154436	2	408391	13	NULL	NULL	0	NULL	United States of America	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The President of the United States of America : a neglected person in our emergency medical system .
	manualset3
154437	3	408391	13	NULL	NULL	0	NULL	person	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The President of the United States of America : a neglected person in our emergency medical system .
	manualset3
154438	4	408391	13	NULL	NULL	0	NULL	emergency medical system	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The President of the United States of America : a neglected person in our emergency medical system .
	manualset3
154440	1	408392	13	NULL	NULL	0	NULL	Programme	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Programme aims to develop human resources and to improve the quality of life of the population , using life expectancy , access to primary health care , and literacy as indicators of quality of life .
	manualset3
154441	2	408392	13	NULL	NULL	0	NULL	aims	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Programme aims to develop human resources and to improve the quality of life of the population , using life expectancy , access to primary health care , and literacy as indicators of quality of life .
	manualset3
154442	3	408392	13	NULL	NULL	0	NULL	human resources 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The Programme aims to develop human resources and to improve the quality of life of the population , using life expectancy , access to primary health care , and literacy as indicators of quality of life .
	manualset3
154443	4	408392	13	NULL	NULL	0	NULL	quality of life 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Programme aims to develop human resources and to improve the quality of life of the population , using life expectancy , access to primary health care , and literacy as indicators of quality of life .
	manualset3
154444	5	408392	13	NULL	NULL	0	NULL	population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The Programme aims to develop human resources and to improve the quality of life of the population , using life expectancy , access to primary health care , and literacy as indicators of quality of life .
	manualset3
154445	6	408392	13	NULL	NULL	NULL	NULL	life expectancy 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The Programme aims to develop human resources and to improve the quality of life of the population , using life expectancy , access to primary health care , and literacy as indicators of quality of life .
	manualset3
154446	7	408392	13	NULL	NULL	0	NULL	access 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Programme aims to develop human resources and to improve the quality of life of the population , using life expectancy , access to primary health care , and literacy as indicators of quality of life .
	manualset3
154447	8	408392	13	NULL	NULL	0	NULL	primary health care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The Programme aims to develop human resources and to improve the quality of life of the population , using life expectancy , access to primary health care , and literacy as indicators of quality of life .
	manualset3
154448	9	408392	13	NULL	NULL	0	NULL	literacy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Programme aims to develop human resources and to improve the quality of life of the population , using life expectancy , access to primary health care , and literacy as indicators of quality of life .
	manualset3
154449	10	408392	13	NULL	NULL	0	NULL	indicators 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Programme aims to develop human resources and to improve the quality of life of the population , using life expectancy , access to primary health care , and literacy as indicators of quality of life .
	manualset3
154450	11	408392	13	NULL	NULL	0	NULL	quality of life	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Programme aims to develop human resources and to improve the quality of life of the population , using life expectancy , access to primary health care , and literacy as indicators of quality of life .
	manualset3
154451	1	408393	13	NULL	NULL	NULL	NULL	Protein Misfolding Cyclic Amplification ( PMCA ) 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The Protein Misfolding Cyclic Amplification ( PMCA ) , a process consisting of sonication and incubation , is one of the few methods thought to model autocatalytic prion replication and generation of proteinase K ( PK ) - resistant PrP ( PrPres ) in vitro .
	manualset3
154452	2	408393	13	NULL	NULL	0	NULL	process 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Protein Misfolding Cyclic Amplification ( PMCA ) , a process consisting of sonication and incubation , is one of the few methods thought to model autocatalytic prion replication and generation of proteinase K ( PK ) - resistant PrP ( PrPres ) in vitro .
	manualset3
154453	3	408393	13	NULL	NULL	0	NULL	sonication 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Protein Misfolding Cyclic Amplification ( PMCA ) , a process consisting of sonication and incubation , is one of the few methods thought to model autocatalytic prion replication and generation of proteinase K ( PK ) - resistant PrP ( PrPres ) in vitro .
	manualset3
154454	4	408393	13	NULL	NULL	0	NULL	incubation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Protein Misfolding Cyclic Amplification ( PMCA ) , a process consisting of sonication and incubation , is one of the few methods thought to model autocatalytic prion replication and generation of proteinase K ( PK ) - resistant PrP ( PrPres ) in vitro .
	manualset3
154455	5	408393	13	NULL	NULL	0	NULL	methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Protein Misfolding Cyclic Amplification ( PMCA ) , a process consisting of sonication and incubation , is one of the few methods thought to model autocatalytic prion replication and generation of proteinase K ( PK ) - resistant PrP ( PrPres ) in vitro .
	manualset3
154456	6	408393	13	NULL	NULL	0	NULL	model 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Protein Misfolding Cyclic Amplification ( PMCA ) , a process consisting of sonication and incubation , is one of the few methods thought to model autocatalytic prion replication and generation of proteinase K ( PK ) - resistant PrP ( PrPres ) in vitro .
	manualset3
154457	7	408393	13	NULL	NULL	0	NULL	autocatalytic prion replication 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Protein Misfolding Cyclic Amplification ( PMCA ) , a process consisting of sonication and incubation , is one of the few methods thought to model autocatalytic prion replication and generation of proteinase K ( PK ) - resistant PrP ( PrPres ) in vitro .
	manualset3
154458	8	408393	13	NULL	NULL	0	NULL	generation of proteinase K ( PK ) - resistant PrP ( PrPres ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Protein Misfolding Cyclic Amplification ( PMCA ) , a process consisting of sonication and incubation , is one of the few methods thought to model autocatalytic prion replication and generation of proteinase K ( PK ) - resistant PrP ( PrPres ) in vitro .
	manualset3
154459	1	408394	13	NULL	NULL	0	NULL	Pt substrates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The Pt substrates can be repeatedly used for graphene growth .
	manualset3
154460	2	408394	13	NULL	NULL	0	NULL	graphene growth	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Pt substrates can be repeatedly used for graphene growth .
	manualset3
154461	1	408395	13	NULL	NULL	0	NULL	compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A related compound , vitamin D2 , could be also converted to 25-hydroxyvitamin D2 and 1 alpha , 25-dihydroxyvitamin D2 using the same strain .
	manualset3
154462	2	408395	13	NULL	NULL	0	NULL	vitamin D2	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A related compound , vitamin D2 , could be also converted to 25-hydroxyvitamin D2 and 1 alpha , 25-dihydroxyvitamin D2 using the same strain .
	manualset3
154463	3	408395	13	NULL	NULL	0	NULL	25-hydroxyvitamin D2 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A related compound , vitamin D2 , could be also converted to 25-hydroxyvitamin D2 and 1 alpha , 25-dihydroxyvitamin D2 using the same strain .
	manualset3
154464	4	408395	13	NULL	NULL	0	NULL	1 alpha , 25-dihydroxyvitamin D2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A related compound , vitamin D2 , could be also converted to 25-hydroxyvitamin D2 and 1 alpha , 25-dihydroxyvitamin D2 using the same strain .
	manualset3
154465	5	408395	13	NULL	NULL	0	NULL	strain 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A related compound , vitamin D2 , could be also converted to 25-hydroxyvitamin D2 and 1 alpha , 25-dihydroxyvitamin D2 using the same strain .
	manualset3
154466	1	408396	13	NULL	NULL	0	NULL	QRS duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The QRS duration , QTc , and JT intervals on 12 lead surface ECG before administration of these drugs were all within normal range .
	manualset3
154467	2	408396	13	NULL	NULL	0	NULL	QTc	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The QRS duration , QTc , and JT intervals on 12 lead surface ECG before administration of these drugs were all within normal range .
	manualset3
154468	3	408396	13	NULL	NULL	0	NULL	JT intervals	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The QRS duration , QTc , and JT intervals on 12 lead surface ECG before administration of these drugs were all within normal range .
	manualset3
154469	4	408396	13	NULL	NULL	0	NULL	12 lead surface ECG	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The QRS duration , QTc , and JT intervals on 12 lead surface ECG before administration of these drugs were all within normal range .
	manualset3
154470	5	408396	13	NULL	NULL	0	NULL	administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The QRS duration , QTc , and JT intervals on 12 lead surface ECG before administration of these drugs were all within normal range .
	manualset3
154471	6	408396	13	NULL	NULL	0	NULL	drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The QRS duration , QTc , and JT intervals on 12 lead surface ECG before administration of these drugs were all within normal range .
	manualset3
154472	7	408396	13	NULL	NULL	0	NULL	normal range	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The QRS duration , QTc , and JT intervals on 12 lead surface ECG before administration of these drugs were all within normal range .
	manualset3
154473	1	408397	13	NULL	NULL	0	NULL	RAD51 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The RAD51 protein has been shown to participate in homologous recombination by promoting ATP-dependent homologous pairing and strand transfer reactions .
	manualset3
154474	2	408397	13	NULL	NULL	0	NULL	homologous recombination 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The RAD51 protein has been shown to participate in homologous recombination by promoting ATP-dependent homologous pairing and strand transfer reactions .
	manualset3
154475	3	408397	13	NULL	NULL	0	NULL	ATP-dependent homologous pairing	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The RAD51 protein has been shown to participate in homologous recombination by promoting ATP-dependent homologous pairing and strand transfer reactions .
	manualset3
154476	4	408397	13	NULL	NULL	0	NULL	strand transfer reactions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The RAD51 protein has been shown to participate in homologous recombination by promoting ATP-dependent homologous pairing and strand transfer reactions .
	manualset3
154477	1	408398	13	NULL	NULL	0	NULL	RAIU 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The RAIU of lactating mammary gland was partially inhibited by treatment with a selective oxytocin antagonist or bromocriptine , an inhibitor of PRL release .
	manualset3
154478	2	408398	13	NULL	NULL	0	NULL	lactating mammary gland	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The RAIU of lactating mammary gland was partially inhibited by treatment with a selective oxytocin antagonist or bromocriptine , an inhibitor of PRL release .
	manualset3
154479	3	408398	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The RAIU of lactating mammary gland was partially inhibited by treatment with a selective oxytocin antagonist or bromocriptine , an inhibitor of PRL release .
	manualset3
154480	4	408398	13	NULL	NULL	0	NULL	selective oxytocin antagonist 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The RAIU of lactating mammary gland was partially inhibited by treatment with a selective oxytocin antagonist or bromocriptine , an inhibitor of PRL release .
	manualset3
154481	5	408398	13	NULL	NULL	0	NULL	bromocriptine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The RAIU of lactating mammary gland was partially inhibited by treatment with a selective oxytocin antagonist or bromocriptine , an inhibitor of PRL release .
	manualset3
154482	6	408398	13	NULL	NULL	0	NULL	inhibitor 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The RAIU of lactating mammary gland was partially inhibited by treatment with a selective oxytocin antagonist or bromocriptine , an inhibitor of PRL release .
	manualset3
154483	7	408398	13	NULL	NULL	0	NULL	PRL release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The RAIU of lactating mammary gland was partially inhibited by treatment with a selective oxytocin antagonist or bromocriptine , an inhibitor of PRL release .
	manualset3
154484	1	408399	13	NULL	NULL	0	NULL	RAST results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The RAST results correlated well with the results of skin prick tests to felt and castor bean extracts .
	manualset3
154485	2	408399	13	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The RAST results correlated well with the results of skin prick tests to felt and castor bean extracts .
	manualset3
154486	3	408399	13	NULL	NULL	0	NULL	skin prick tests 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The RAST results correlated well with the results of skin prick tests to felt and castor bean extracts .
	manualset3
154487	4	408399	13	NULL	NULL	0	NULL	felt extracts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The RAST results correlated well with the results of skin prick tests to felt and castor bean extracts .
	manualset3
154488	5	408399	13	NULL	NULL	0	NULL	castor bean extracts 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The RAST results correlated well with the results of skin prick tests to felt and castor bean extracts .
	manualset3
154489	1	408400	13	NULL	NULL	0	NULL	RFLP profiles	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The RFLP profiles seen in Maryland , Ohio , Massachusetts , and New York ATCC strains were identical to those of some Mississippi isolates , even though the samples were isolated 10-35 years apart .
	manualset3
154490	2	408400	13	NULL	NULL	0	NULL	Maryland	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The RFLP profiles seen in Maryland , Ohio , Massachusetts , and New York ATCC strains were identical to those of some Mississippi isolates , even though the samples were isolated 10-35 years apart .
	manualset3
154491	3	408400	13	NULL	NULL	0	NULL	Ohio 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The RFLP profiles seen in Maryland , Ohio , Massachusetts , and New York ATCC strains were identical to those of some Mississippi isolates , even though the samples were isolated 10-35 years apart .
	manualset3
154492	4	408400	13	NULL	NULL	0	NULL	Massachusetts	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The RFLP profiles seen in Maryland , Ohio , Massachusetts , and New York ATCC strains were identical to those of some Mississippi isolates , even though the samples were isolated 10-35 years apart .
	manualset3
154493	5	408400	13	NULL	NULL	0	NULL	New York	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The RFLP profiles seen in Maryland , Ohio , Massachusetts , and New York ATCC strains were identical to those of some Mississippi isolates , even though the samples were isolated 10-35 years apart .
	manualset3
154494	6	408400	13	NULL	NULL	0	NULL	ATCC strains 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The RFLP profiles seen in Maryland , Ohio , Massachusetts , and New York ATCC strains were identical to those of some Mississippi isolates , even though the samples were isolated 10-35 years apart .
	manualset3
154495	7	408400	13	NULL	NULL	0	NULL	Mississippi isolates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The RFLP profiles seen in Maryland , Ohio , Massachusetts , and New York ATCC strains were identical to those of some Mississippi isolates , even though the samples were isolated 10-35 years apart .
	manualset3
154496	8	408400	13	NULL	NULL	0	NULL	samples 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The RFLP profiles seen in Maryland , Ohio , Massachusetts , and New York ATCC strains were identical to those of some Mississippi isolates , even though the samples were isolated 10-35 years apart .
	manualset3
154497	9	408400	13	NULL	NULL	0	NULL	10-35 years apart	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The RFLP profiles seen in Maryland , Ohio , Massachusetts , and New York ATCC strains were identical to those of some Mississippi isolates , even though the samples were isolated 10-35 years apart .
	manualset3
154498	1	408401	13	NULL	NULL	0	NULL	RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The RNA encoded by the 3 ' untranslated region of the prohibitin gene arrests cell proliferation by blocking the transition between the G1 and S phases of the cell cycle .
	manualset3
154499	2	408401	13	NULL	NULL	0	NULL	3 ' untranslated region 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The RNA encoded by the 3 ' untranslated region of the prohibitin gene arrests cell proliferation by blocking the transition between the G1 and S phases of the cell cycle .
	manualset3
154500	3	408401	13	NULL	NULL	0	NULL	prohibitin gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The RNA encoded by the 3 ' untranslated region of the prohibitin gene arrests cell proliferation by blocking the transition between the G1 and S phases of the cell cycle .
	manualset3
154501	4	408401	13	NULL	NULL	0	NULL	arrests 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The RNA encoded by the 3 ' untranslated region of the prohibitin gene arrests cell proliferation by blocking the transition between the G1 and S phases of the cell cycle .
	manualset3
154502	5	408401	13	NULL	NULL	0	NULL	cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The RNA encoded by the 3 ' untranslated region of the prohibitin gene arrests cell proliferation by blocking the transition between the G1 and S phases of the cell cycle .
	manualset3
154503	6	408401	13	NULL	NULL	0	NULL	transition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The RNA encoded by the 3 ' untranslated region of the prohibitin gene arrests cell proliferation by blocking the transition between the G1 and S phases of the cell cycle .
	manualset3
154504	7	408401	13	NULL	NULL	0	NULL	G1 phase	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The RNA encoded by the 3 ' untranslated region of the prohibitin gene arrests cell proliferation by blocking the transition between the G1 and S phases of the cell cycle .
	manualset3
154505	8	408401	13	NULL	NULL	0	NULL	S phase	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The RNA encoded by the 3 ' untranslated region of the prohibitin gene arrests cell proliferation by blocking the transition between the G1 and S phases of the cell cycle .
	manualset3
154506	9	408401	13	NULL	NULL	0	NULL	cell cycle	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The RNA encoded by the 3 ' untranslated region of the prohibitin gene arrests cell proliferation by blocking the transition between the G1 and S phases of the cell cycle .
	manualset3
154507	1	408402	13	NULL	NULL	0	NULL	RNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The RNA is 11 , 835 nucleotides in length and the organization of the genome is typical of alphaviruses .
	manualset3
154508	2	408402	13	NULL	NULL	0	NULL	11 , 835 nucleotides	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The RNA is 11 , 835 nucleotides in length and the organization of the genome is typical of alphaviruses .
	manualset3
154509	3	408402	13	NULL	NULL	0	NULL	length	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The RNA is 11 , 835 nucleotides in length and the organization of the genome is typical of alphaviruses .
	manualset3
154510	4	408402	13	NULL	NULL	0	NULL	organization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The RNA is 11 , 835 nucleotides in length and the organization of the genome is typical of alphaviruses .
	manualset3
154511	5	408402	13	NULL	NULL	0	NULL	genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The RNA is 11 , 835 nucleotides in length and the organization of the genome is typical of alphaviruses .
	manualset3
154512	6	408402	13	NULL	NULL	0	NULL	alphaviruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The RNA is 11 , 835 nucleotides in length and the organization of the genome is typical of alphaviruses .
	manualset3
154513	1	408403	13	NULL	NULL	0	NULL	Ras cascade functions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Ras cascade functions in other Drosophila signal transduction pathways , eliciting a distinct response in each case , presumably through phosphorylation of specific transcription factors .
	manualset3
154514	2	408403	13	NULL	NULL	0	NULL	Drosophila signal transduction pathways 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Ras cascade functions in other Drosophila signal transduction pathways , eliciting a distinct response in each case , presumably through phosphorylation of specific transcription factors .
	manualset3
154515	3	408403	13	NULL	NULL	0	NULL	response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Ras cascade functions in other Drosophila signal transduction pathways , eliciting a distinct response in each case , presumably through phosphorylation of specific transcription factors .
	manualset3
154516	4	408403	13	NULL	NULL	0	NULL	case	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Ras cascade functions in other Drosophila signal transduction pathways , eliciting a distinct response in each case , presumably through phosphorylation of specific transcription factors .
	manualset3
154517	5	408403	13	NULL	NULL	0	NULL	phosphorylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Ras cascade functions in other Drosophila signal transduction pathways , eliciting a distinct response in each case , presumably through phosphorylation of specific transcription factors .
	manualset3
154518	6	408403	13	NULL	NULL	0	NULL	specific transcription factors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The Ras cascade functions in other Drosophila signal transduction pathways , eliciting a distinct response in each case , presumably through phosphorylation of specific transcription factors .
	manualset3
154519	1	408404	13	NULL	NULL	0	NULL	Registry 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Registry continues to work both in the field of end-stage renal failure and other fields of renal disease .
	manualset3
154520	2	408404	13	NULL	NULL	0	NULL	field of end-stage renal failure 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The Registry continues to work both in the field of end-stage renal failure and other fields of renal disease .
	manualset3
154521	3	408404	13	NULL	NULL	0	NULL	fields of renal disease	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The Registry continues to work both in the field of end-stage renal failure and other fields of renal disease .
	manualset3
154522	1	408405	13	NULL	NULL	0	NULL	Registry	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Registry is designed to ( 1 ) promote the continuing care of the patient , ( 2 ) to evaluate cancer control methods , ( 3 ) to advance knowledge of the epidemiology of cancer , and ( 4 ) to suggest leads for laboratory and clinical research .
	manualset3
154523	2	408405	13	NULL	NULL	0	NULL	care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The Registry is designed to ( 1 ) promote the continuing care of the patient , ( 2 ) to evaluate cancer control methods , ( 3 ) to advance knowledge of the epidemiology of cancer , and ( 4 ) to suggest leads for laboratory and clinical research .
	manualset3
154524	3	408405	13	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The Registry is designed to ( 1 ) promote the continuing care of the patient , ( 2 ) to evaluate cancer control methods , ( 3 ) to advance knowledge of the epidemiology of cancer , and ( 4 ) to suggest leads for laboratory and clinical research .
	manualset3
154525	4	408405	13	NULL	NULL	0	NULL	cancer control methods	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The Registry is designed to ( 1 ) promote the continuing care of the patient , ( 2 ) to evaluate cancer control methods , ( 3 ) to advance knowledge of the epidemiology of cancer , and ( 4 ) to suggest leads for laboratory and clinical research .
	manualset3
154526	5	408405	13	NULL	NULL	0	NULL	knowledge	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The Registry is designed to ( 1 ) promote the continuing care of the patient , ( 2 ) to evaluate cancer control methods , ( 3 ) to advance knowledge of the epidemiology of cancer , and ( 4 ) to suggest leads for laboratory and clinical research .
	manualset3
154527	6	408405	13	NULL	NULL	0	NULL	epidemiology of cancer 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Registry is designed to ( 1 ) promote the continuing care of the patient , ( 2 ) to evaluate cancer control methods , ( 3 ) to advance knowledge of the epidemiology of cancer , and ( 4 ) to suggest leads for laboratory and clinical research .
	manualset3
154528	7	408405	13	NULL	NULL	0	NULL	laboratory	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The Registry is designed to ( 1 ) promote the continuing care of the patient , ( 2 ) to evaluate cancer control methods , ( 3 ) to advance knowledge of the epidemiology of cancer , and ( 4 ) to suggest leads for laboratory and clinical research .
	manualset3
154529	8	408405	13	NULL	NULL	0	NULL	clinical research 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Registry is designed to ( 1 ) promote the continuing care of the patient , ( 2 ) to evaluate cancer control methods , ( 3 ) to advance knowledge of the epidemiology of cancer , and ( 4 ) to suggest leads for laboratory and clinical research .
	manualset3
154530	1	408406	13	NULL	NULL	0	NULL	Rfc-Rol-dependent pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Rfc-Rol-dependent pathway for O-antigen synthesis is found in strains with heteropolysaccharide O antigens , and , consistent with this association , rol-homologous sequences were detected in chromosomal DNAs from 17 different serotypes with heteropolysaccharide O antigens .
	manualset3
154531	2	408406	13	NULL	NULL	0	NULL	O-antigen synthesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Rfc-Rol-dependent pathway for O-antigen synthesis is found in strains with heteropolysaccharide O antigens , and , consistent with this association , rol-homologous sequences were detected in chromosomal DNAs from 17 different serotypes with heteropolysaccharide O antigens .
	manualset3
154532	3	408406	13	NULL	NULL	0	NULL	strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The Rfc-Rol-dependent pathway for O-antigen synthesis is found in strains with heteropolysaccharide O antigens , and , consistent with this association , rol-homologous sequences were detected in chromosomal DNAs from 17 different serotypes with heteropolysaccharide O antigens .
	manualset3
154533	4	408406	13	NULL	NULL	0	NULL	heteropolysaccharide O antigens 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The Rfc-Rol-dependent pathway for O-antigen synthesis is found in strains with heteropolysaccharide O antigens , and , consistent with this association , rol-homologous sequences were detected in chromosomal DNAs from 17 different serotypes with heteropolysaccharide O antigens .
	manualset3
154534	5	408406	13	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The Rfc-Rol-dependent pathway for O-antigen synthesis is found in strains with heteropolysaccharide O antigens , and , consistent with this association , rol-homologous sequences were detected in chromosomal DNAs from 17 different serotypes with heteropolysaccharide O antigens .
	manualset3
154535	6	408406	13	NULL	NULL	0	NULL	rol-homologous sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The Rfc-Rol-dependent pathway for O-antigen synthesis is found in strains with heteropolysaccharide O antigens , and , consistent with this association , rol-homologous sequences were detected in chromosomal DNAs from 17 different serotypes with heteropolysaccharide O antigens .
	manualset3
154536	7	408406	13	NULL	NULL	0	NULL	chromosomal DNAs 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The Rfc-Rol-dependent pathway for O-antigen synthesis is found in strains with heteropolysaccharide O antigens , and , consistent with this association , rol-homologous sequences were detected in chromosomal DNAs from 17 different serotypes with heteropolysaccharide O antigens .
	manualset3
154537	8	408406	13	NULL	NULL	0	NULL	17 different serotypes 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Rfc-Rol-dependent pathway for O-antigen synthesis is found in strains with heteropolysaccharide O antigens , and , consistent with this association , rol-homologous sequences were detected in chromosomal DNAs from 17 different serotypes with heteropolysaccharide O antigens .
	manualset3
154538	9	408406	13	NULL	NULL	0	NULL	heteropolysaccharide O antigens 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The Rfc-Rol-dependent pathway for O-antigen synthesis is found in strains with heteropolysaccharide O antigens , and , consistent with this association , rol-homologous sequences were detected in chromosomal DNAs from 17 different serotypes with heteropolysaccharide O antigens .
	manualset3
154539	1	408407	13	NULL	NULL	0	NULL	Rho family of GTP binding proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The Rho family of GTP binding proteins are important upstream mediators of cytoskeletal organization .
	manualset3
154540	2	408407	13	NULL	NULL	0	NULL	upstream mediators	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The Rho family of GTP binding proteins are important upstream mediators of cytoskeletal organization .
	manualset3
154541	3	408407	13	NULL	NULL	0	NULL	cytoskeletal organization 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Rho family of GTP binding proteins are important upstream mediators of cytoskeletal organization .
	manualset3
154542	1	408408	13	NULL	NULL	0	NULL	Rho family of GTPases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The Rho family of GTPases regulates many aspects of cellular behavior through alterations to the actin cytoskeleton , acting as molecular switches cycling between the active , GTP-bound and the inactive , GDP-bound conformations .
	manualset3
154543	2	408408	13	NULL	NULL	0	NULL	aspects of cellular behavior 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Rho family of GTPases regulates many aspects of cellular behavior through alterations to the actin cytoskeleton , acting as molecular switches cycling between the active , GTP-bound and the inactive , GDP-bound conformations .
	manualset3
154544	3	408408	13	NULL	NULL	0	NULL	alterations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Rho family of GTPases regulates many aspects of cellular behavior through alterations to the actin cytoskeleton , acting as molecular switches cycling between the active , GTP-bound and the inactive , GDP-bound conformations .
	manualset3
154545	4	408408	13	NULL	NULL	0	NULL	actin cytoskeleton	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The Rho family of GTPases regulates many aspects of cellular behavior through alterations to the actin cytoskeleton , acting as molecular switches cycling between the active , GTP-bound and the inactive , GDP-bound conformations .
	manualset3
154546	5	408408	13	NULL	NULL	0	NULL	molecular switches	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Rho family of GTPases regulates many aspects of cellular behavior through alterations to the actin cytoskeleton , acting as molecular switches cycling between the active , GTP-bound and the inactive , GDP-bound conformations .
	manualset3
154547	6	408408	13	NULL	NULL	0	NULL	active , GTP-bound conformations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Rho family of GTPases regulates many aspects of cellular behavior through alterations to the actin cytoskeleton , acting as molecular switches cycling between the active , GTP-bound and the inactive , GDP-bound conformations .
	manualset3
154548	7	408408	13	NULL	NULL	0	NULL	inactive , GDP-bound conformations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Rho family of GTPases regulates many aspects of cellular behavior through alterations to the actin cytoskeleton , acting as molecular switches cycling between the active , GTP-bound and the inactive , GDP-bound conformations .
	manualset3
154549	1	408409	13	NULL	NULL	0	NULL	Royal Society of London	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The Royal Society of London held a scientific meeting in September 2000 focusing on two theories of the origin of AIDS : one , that it occurred through `` natural transfer '' of immunodeficiency virus from monkeys or chimpanzees to humans ; and the other , that it occurred through iatrogenic transfer via contaminated polio vaccines used in Africa in the late 1950s .
	manualset3
154550	2	408409	13	NULL	NULL	0	NULL	scientific meeting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Royal Society of London held a scientific meeting in September 2000 focusing on two theories of the origin of AIDS : one , that it occurred through `` natural transfer '' of immunodeficiency virus from monkeys or chimpanzees to humans ; and the other , that it occurred through iatrogenic transfer via contaminated polio vaccines used in Africa in the late 1950s .
	manualset3
154551	3	408409	13	NULL	NULL	0	NULL	September 2000	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The Royal Society of London held a scientific meeting in September 2000 focusing on two theories of the origin of AIDS : one , that it occurred through `` natural transfer '' of immunodeficiency virus from monkeys or chimpanzees to humans ; and the other , that it occurred through iatrogenic transfer via contaminated polio vaccines used in Africa in the late 1950s .
	manualset3
154552	4	408409	13	NULL	NULL	0	NULL	focusing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Royal Society of London held a scientific meeting in September 2000 focusing on two theories of the origin of AIDS : one , that it occurred through `` natural transfer '' of immunodeficiency virus from monkeys or chimpanzees to humans ; and the other , that it occurred through iatrogenic transfer via contaminated polio vaccines used in Africa in the late 1950s .
	manualset3
154553	5	408409	13	NULL	NULL	0	NULL	two theories	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The Royal Society of London held a scientific meeting in September 2000 focusing on two theories of the origin of AIDS : one , that it occurred through `` natural transfer '' of immunodeficiency virus from monkeys or chimpanzees to humans ; and the other , that it occurred through iatrogenic transfer via contaminated polio vaccines used in Africa in the late 1950s .
	manualset3
154554	6	408409	13	NULL	NULL	0	NULL	origin of AIDS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Royal Society of London held a scientific meeting in September 2000 focusing on two theories of the origin of AIDS : one , that it occurred through `` natural transfer '' of immunodeficiency virus from monkeys or chimpanzees to humans ; and the other , that it occurred through iatrogenic transfer via contaminated polio vaccines used in Africa in the late 1950s .
	manualset3
154555	7	408409	13	NULL	NULL	0	NULL	natural transfer	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Royal Society of London held a scientific meeting in September 2000 focusing on two theories of the origin of AIDS : one , that it occurred through `` natural transfer '' of immunodeficiency virus from monkeys or chimpanzees to humans ; and the other , that it occurred through iatrogenic transfer via contaminated polio vaccines used in Africa in the late 1950s .
	manualset3
154556	8	408409	13	NULL	NULL	0	NULL	immunodeficiency virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The Royal Society of London held a scientific meeting in September 2000 focusing on two theories of the origin of AIDS : one , that it occurred through `` natural transfer '' of immunodeficiency virus from monkeys or chimpanzees to humans ; and the other , that it occurred through iatrogenic transfer via contaminated polio vaccines used in Africa in the late 1950s .
	manualset3
154557	9	408409	13	NULL	NULL	0	NULL	monkeys 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The Royal Society of London held a scientific meeting in September 2000 focusing on two theories of the origin of AIDS : one , that it occurred through `` natural transfer '' of immunodeficiency virus from monkeys or chimpanzees to humans ; and the other , that it occurred through iatrogenic transfer via contaminated polio vaccines used in Africa in the late 1950s .
	manualset3
154558	10	408409	13	NULL	NULL	0	NULL	chimpanzees	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The Royal Society of London held a scientific meeting in September 2000 focusing on two theories of the origin of AIDS : one , that it occurred through `` natural transfer '' of immunodeficiency virus from monkeys or chimpanzees to humans ; and the other , that it occurred through iatrogenic transfer via contaminated polio vaccines used in Africa in the late 1950s .
	manualset3
154559	11	408409	13	NULL	NULL	0	NULL	humans 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The Royal Society of London held a scientific meeting in September 2000 focusing on two theories of the origin of AIDS : one , that it occurred through `` natural transfer '' of immunodeficiency virus from monkeys or chimpanzees to humans ; and the other , that it occurred through iatrogenic transfer via contaminated polio vaccines used in Africa in the late 1950s .
	manualset3
154560	12	408409	13	NULL	NULL	0	NULL	iatrogenic transfer 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Royal Society of London held a scientific meeting in September 2000 focusing on two theories of the origin of AIDS : one , that it occurred through `` natural transfer '' of immunodeficiency virus from monkeys or chimpanzees to humans ; and the other , that it occurred through iatrogenic transfer via contaminated polio vaccines used in Africa in the late 1950s .
	manualset3
154561	13	408409	13	NULL	NULL	0	NULL	polio vaccines	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The Royal Society of London held a scientific meeting in September 2000 focusing on two theories of the origin of AIDS : one , that it occurred through `` natural transfer '' of immunodeficiency virus from monkeys or chimpanzees to humans ; and the other , that it occurred through iatrogenic transfer via contaminated polio vaccines used in Africa in the late 1950s .
	manualset3
154562	14	408409	13	NULL	NULL	0	NULL	Africa 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The Royal Society of London held a scientific meeting in September 2000 focusing on two theories of the origin of AIDS : one , that it occurred through `` natural transfer '' of immunodeficiency virus from monkeys or chimpanzees to humans ; and the other , that it occurred through iatrogenic transfer via contaminated polio vaccines used in Africa in the late 1950s .
	manualset3
154563	15	408409	13	NULL	NULL	0	NULL	late 1950s	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The Royal Society of London held a scientific meeting in September 2000 focusing on two theories of the origin of AIDS : one , that it occurred through `` natural transfer '' of immunodeficiency virus from monkeys or chimpanzees to humans ; and the other , that it occurred through iatrogenic transfer via contaminated polio vaccines used in Africa in the late 1950s .
	manualset3
154564	1	408410	13	NULL	NULL	0	NULL	Rv	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Rv of the normal group was 5.06 + / - 1.53 whereas the Rv of the silica treated group was 2.13 + / - 1.20 .
	manualset3
154565	2	408410	13	NULL	NULL	0	NULL	normal group 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The Rv of the normal group was 5.06 + / - 1.53 whereas the Rv of the silica treated group was 2.13 + / - 1.20 .
	manualset3
154566	3	408410	13	NULL	NULL	0	NULL	5.06 + / - 1.53	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Rv of the normal group was 5.06 + / - 1.53 whereas the Rv of the silica treated group was 2.13 + / - 1.20 .
	manualset3
154567	4	408410	13	NULL	NULL	0	NULL	Rv 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Rv of the normal group was 5.06 + / - 1.53 whereas the Rv of the silica treated group was 2.13 + / - 1.20 .
	manualset3
154568	5	408410	13	NULL	NULL	0	NULL	silica treated group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The Rv of the normal group was 5.06 + / - 1.53 whereas the Rv of the silica treated group was 2.13 + / - 1.20 .
	manualset3
154569	6	408410	13	NULL	NULL	0	NULL	2.13 + / - 1.20	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Rv of the normal group was 5.06 + / - 1.53 whereas the Rv of the silica treated group was 2.13 + / - 1.20 .
	manualset3
154570	1	408411	13	NULL	NULL	0	NULL	S-S bond 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The S-S bond elongates to 2.054 Angstroms , while the S-O bond shortens from 1.755 Angstroms in neutral form to 1.684 Angstroms in its corresponding cationic-radical form .
	manualset3
154571	2	408411	13	NULL	NULL	0	NULL	2.054 Angstroms	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The S-S bond elongates to 2.054 Angstroms , while the S-O bond shortens from 1.755 Angstroms in neutral form to 1.684 Angstroms in its corresponding cationic-radical form .
	manualset3
154572	3	408411	13	NULL	NULL	0	NULL	S-O bond	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The S-S bond elongates to 2.054 Angstroms , while the S-O bond shortens from 1.755 Angstroms in neutral form to 1.684 Angstroms in its corresponding cationic-radical form .
	manualset3
154574	5	408411	13	NULL	NULL	0	NULL	1.755 Angstroms 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The S-S bond elongates to 2.054 Angstroms , while the S-O bond shortens from 1.755 Angstroms in neutral form to 1.684 Angstroms in its corresponding cationic-radical form .
	manualset3
154575	6	408411	13	NULL	NULL	0	NULL	neutral form	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The S-S bond elongates to 2.054 Angstroms , while the S-O bond shortens from 1.755 Angstroms in neutral form to 1.684 Angstroms in its corresponding cationic-radical form .
	manualset3
154576	7	408411	13	NULL	NULL	0	NULL	1.684 Angstroms 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The S-S bond elongates to 2.054 Angstroms , while the S-O bond shortens from 1.755 Angstroms in neutral form to 1.684 Angstroms in its corresponding cationic-radical form .
	manualset3
154577	8	408411	13	NULL	NULL	0	NULL	cationic-radical form	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The S-S bond elongates to 2.054 Angstroms , while the S-O bond shortens from 1.755 Angstroms in neutral form to 1.684 Angstroms in its corresponding cationic-radical form .
	manualset3
154578	1	408412	13	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A relationship between accumulations of PAH compounds in Hypnum cupressiforme and octanol-air partition coefficients was obtained and is briefly discussed .
	manualset3
154579	2	408412	13	NULL	NULL	0	NULL	accumulations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A relationship between accumulations of PAH compounds in Hypnum cupressiforme and octanol-air partition coefficients was obtained and is briefly discussed .
	manualset3
154580	3	408412	13	NULL	NULL	0	NULL	PAH compounds 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A relationship between accumulations of PAH compounds in Hypnum cupressiforme and octanol-air partition coefficients was obtained and is briefly discussed .
	manualset3
154581	4	408412	13	NULL	NULL	0	NULL	Hypnum cupressiforme	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A relationship between accumulations of PAH compounds in Hypnum cupressiforme and octanol-air partition coefficients was obtained and is briefly discussed .
	manualset3
154582	5	408412	13	NULL	NULL	0	NULL	octanol-air partition coefficients	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A relationship between accumulations of PAH compounds in Hypnum cupressiforme and octanol-air partition coefficients was obtained and is briefly discussed .
	manualset3
154583	1	408413	13	NULL	NULL	0	NULL	S. equorum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The S. equorum sequence diversity showed at the intra-species level by recA gene sequencing confirmed the high heterogeneity described among S. equorum strains .
	manualset3
154584	2	408413	13	NULL	NULL	0	NULL	sequence diversity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The S. equorum sequence diversity showed at the intra-species level by recA gene sequencing confirmed the high heterogeneity described among S. equorum strains .
	manualset3
154585	3	408413	13	NULL	NULL	0	NULL	intra-species level	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The S. equorum sequence diversity showed at the intra-species level by recA gene sequencing confirmed the high heterogeneity described among S. equorum strains .
	manualset3
154586	4	408413	13	NULL	NULL	0	NULL	recA gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The S. equorum sequence diversity showed at the intra-species level by recA gene sequencing confirmed the high heterogeneity described among S. equorum strains .
	manualset3
154587	5	408413	13	NULL	NULL	0	NULL	heterogeneity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The S. equorum sequence diversity showed at the intra-species level by recA gene sequencing confirmed the high heterogeneity described among S. equorum strains .
	manualset3
154588	6	408413	13	NULL	NULL	0	NULL	S. equorum strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The S. equorum sequence diversity showed at the intra-species level by recA gene sequencing confirmed the high heterogeneity described among S. equorum strains .
	manualset3
157258	7	408413	13	NULL	NULL	0	NULL	sequencing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The S. equorum sequence diversity showed at the intra-species level by recA gene sequencing confirmed the high heterogeneity described among S. equorum strains .
	manualset3
154589	1	408414	13	NULL	NULL	0	NULL	SG1 antibody 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The SG1 antibody detects a single DNMT3B protein isoform that is expressed only in PSCs but not in SDCs .
	manualset3
154590	2	408414	13	NULL	NULL	0	NULL	DNMT3B protein isoform	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The SG1 antibody detects a single DNMT3B protein isoform that is expressed only in PSCs but not in SDCs .
	manualset3
154591	3	408414	13	NULL	NULL	0	NULL	PSCs	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The SG1 antibody detects a single DNMT3B protein isoform that is expressed only in PSCs but not in SDCs .
	manualset3
154592	4	408414	13	NULL	NULL	0	NULL	SDCs	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The SG1 antibody detects a single DNMT3B protein isoform that is expressed only in PSCs but not in SDCs .
	manualset3
154593	1	408415	13	NULL	NULL	0	NULL	SHERP genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The SHERP genes are found as a tandem pair within the differentially regulated LmcDNA16 locus of Leishmania major .
	manualset3
154594	2	408415	13	NULL	NULL	0	NULL	 tandem pair 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The SHERP genes are found as a tandem pair within the differentially regulated LmcDNA16 locus of Leishmania major .
	manualset3
154595	3	408415	13	NULL	NULL	0	NULL	LmcDNA16 locus 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The SHERP genes are found as a tandem pair within the differentially regulated LmcDNA16 locus of Leishmania major .
	manualset3
154596	4	408415	13	NULL	NULL	0	NULL	Leishmania major	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The SHERP genes are found as a tandem pair within the differentially regulated LmcDNA16 locus of Leishmania major .
	manualset3
154597	1	408416	13	NULL	NULL	0	NULL	SHR 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The SHR seem to be more capable of keeping the myogenic activity in low SBP .
	manualset3
154598	2	408416	13	NULL	NULL	NULL	NULL	myogenic activity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The SHR seem to be more capable of keeping the myogenic activity in low SBP .
	manualset3
154599	3	408416	13	NULL	NULL	0	NULL	low SBP	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The SHR seem to be more capable of keeping the myogenic activity in low SBP .
	manualset3
154600	1	408417	13	NULL	NULL	0	NULL	SHR	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The SHR showed a significantly greater SNA and resultant MAP increase as a function of age compared to that of the WKY rats .
	manualset3
154601	2	408417	13	NULL	NULL	0	NULL	greater SNA	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The SHR showed a significantly greater SNA and resultant MAP increase as a function of age compared to that of the WKY rats .
	manualset3
154602	3	408417	13	NULL	NULL	0	NULL	resultant MAP	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The SHR showed a significantly greater SNA and resultant MAP increase as a function of age compared to that of the WKY rats .
	manualset3
154603	4	408417	13	NULL	NULL	0	NULL	function of age	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The SHR showed a significantly greater SNA and resultant MAP increase as a function of age compared to that of the WKY rats .
	manualset3
154604	5	408417	13	NULL	NULL	0	NULL	WKY rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The SHR showed a significantly greater SNA and resultant MAP increase as a function of age compared to that of the WKY rats .
	manualset3
154605	1	408418	13	NULL	NULL	0	NULL	SNP rs7216389	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The SNP rs7216389 , which tags the 3 ' flanking region of ORMDL3 at 17q21 and has been associated with childhood asthma , was correlated with increased glioma risk ( OR = 1.10 ; 95 % CI : 1.01-1 .19 ) .
	manualset3
154606	2	408418	13	NULL	NULL	0	NULL	3 ' flanking region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The SNP rs7216389 , which tags the 3 ' flanking region of ORMDL3 at 17q21 and has been associated with childhood asthma , was correlated with increased glioma risk ( OR = 1.10 ; 95 % CI : 1.01-1 .19 ) .
	manualset3
154607	3	408418	13	NULL	NULL	0	NULL	ORMDL3 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The SNP rs7216389 , which tags the 3 ' flanking region of ORMDL3 at 17q21 and has been associated with childhood asthma , was correlated with increased glioma risk ( OR = 1.10 ; 95 % CI : 1.01-1 .19 ) .
	manualset3
154608	4	408418	13	NULL	NULL	0	NULL	17q21	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The SNP rs7216389 , which tags the 3 ' flanking region of ORMDL3 at 17q21 and has been associated with childhood asthma , was correlated with increased glioma risk ( OR = 1.10 ; 95 % CI : 1.01-1 .19 ) .
	manualset3
154609	5	408418	13	NULL	NULL	0	NULL	childhood asthma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The SNP rs7216389 , which tags the 3 ' flanking region of ORMDL3 at 17q21 and has been associated with childhood asthma , was correlated with increased glioma risk ( OR = 1.10 ; 95 % CI : 1.01-1 .19 ) .
	manualset3
154610	6	408418	13	NULL	NULL	0	NULL	glioma risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The SNP rs7216389 , which tags the 3 ' flanking region of ORMDL3 at 17q21 and has been associated with childhood asthma , was correlated with increased glioma risk ( OR = 1.10 ; 95 % CI : 1.01-1 .19 ) .
	manualset3
154611	7	408418	13	NULL	NULL	0	NULL	OR = 1.10	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The SNP rs7216389 , which tags the 3 ' flanking region of ORMDL3 at 17q21 and has been associated with childhood asthma , was correlated with increased glioma risk ( OR = 1.10 ; 95 % CI : 1.01-1 .19 ) .
	manualset3
154612	8	408418	13	NULL	NULL	0	NULL	95 % CI : 1.01-1 .19 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The SNP rs7216389 , which tags the 3 ' flanking region of ORMDL3 at 17q21 and has been associated with childhood asthma , was correlated with increased glioma risk ( OR = 1.10 ; 95 % CI : 1.01-1 .19 ) .
	manualset3
154613	1	408419	13	NULL	NULL	0	NULL	SRPN10 dynamics 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The SRPN10 dynamics at the subcellular level confirm and further elaborate the ` time bomb ' model of P. berghei invasion in both Anopheles stephensi and Anopheles gambiae .
	manualset3
154614	2	408419	13	NULL	NULL	0	NULL	subcellular level	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The SRPN10 dynamics at the subcellular level confirm and further elaborate the ` time bomb ' model of P. berghei invasion in both Anopheles stephensi and Anopheles gambiae .
	manualset3
154615	3	408419	13	NULL	NULL	0	NULL	` time bomb ' model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The SRPN10 dynamics at the subcellular level confirm and further elaborate the ` time bomb ' model of P. berghei invasion in both Anopheles stephensi and Anopheles gambiae .
	manualset3
154616	4	408419	13	NULL	NULL	0	NULL	P. berghei	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The SRPN10 dynamics at the subcellular level confirm and further elaborate the ` time bomb ' model of P. berghei invasion in both Anopheles stephensi and Anopheles gambiae .
	manualset3
154617	5	408419	13	NULL	NULL	0	NULL	invasion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The SRPN10 dynamics at the subcellular level confirm and further elaborate the ` time bomb ' model of P. berghei invasion in both Anopheles stephensi and Anopheles gambiae .
	manualset3
154618	6	408419	13	NULL	NULL	0	NULL	Anopheles stephensi 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The SRPN10 dynamics at the subcellular level confirm and further elaborate the ` time bomb ' model of P. berghei invasion in both Anopheles stephensi and Anopheles gambiae .
	manualset3
154619	7	408419	13	NULL	NULL	0	NULL	Anopheles gambiae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The SRPN10 dynamics at the subcellular level confirm and further elaborate the ` time bomb ' model of P. berghei invasion in both Anopheles stephensi and Anopheles gambiae .
	manualset3
154620	1	408420	13	NULL	NULL	0	NULL	ST-353 complex	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The ST-353 complex was the most common complex , whereas the ST-21 , ST-42 , ST-52 , and ST-257 complexes were less well represented .
	manualset3
154621	2	408420	13	NULL	NULL	0	NULL	complex	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The ST-353 complex was the most common complex , whereas the ST-21 , ST-42 , ST-52 , and ST-257 complexes were less well represented .
	manualset3
154622	3	408420	13	NULL	NULL	0	NULL	ST-21 complex	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The ST-353 complex was the most common complex , whereas the ST-21 , ST-42 , ST-52 , and ST-257 complexes were less well represented .
	manualset3
154623	4	408420	13	NULL	NULL	0	NULL	ST-42 complex	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The ST-353 complex was the most common complex , whereas the ST-21 , ST-42 , ST-52 , and ST-257 complexes were less well represented .
	manualset3
154624	5	408420	13	NULL	NULL	0	NULL	ST-52 complex	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The ST-353 complex was the most common complex , whereas the ST-21 , ST-42 , ST-52 , and ST-257 complexes were less well represented .
	manualset3
154625	6	408420	13	NULL	NULL	0	NULL	ST-257 complex	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The ST-353 complex was the most common complex , whereas the ST-21 , ST-42 , ST-52 , and ST-257 complexes were less well represented .
	manualset3
154626	1	408421	13	NULL	NULL	0	NULL	STYK1 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The STYK1 gene is mapped to human chromosome 12p13 and 11 exons were found .
	manualset3
154627	2	408421	13	NULL	NULL	0	NULL	human chromosome 12p13	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The STYK1 gene is mapped to human chromosome 12p13 and 11 exons were found .
	manualset3
154628	3	408421	13	NULL	NULL	0	NULL	11 exons	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The STYK1 gene is mapped to human chromosome 12p13 and 11 exons were found .
	manualset3
154629	1	408422	13	NULL	NULL	0	NULL	relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A relationship was found between bradykinesia and widespread cognitive impairment .
	manualset3
154630	2	408422	13	NULL	NULL	0	NULL	bradykinesia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A relationship was found between bradykinesia and widespread cognitive impairment .
	manualset3
154631	3	408422	13	NULL	NULL	0	NULL	cognitive impairment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A relationship was found between bradykinesia and widespread cognitive impairment .
	manualset3
154632	1	408423	13	NULL	NULL	0	NULL	SVM classification system	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The SVM classification system was further tested on a small class of snRNA-binding proteins with only 60 available sequences .
	manualset3
154633	2	408423	13	NULL	NULL	0	NULL	small class of snRNA-binding proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The SVM classification system was further tested on a small class of snRNA-binding proteins with only 60 available sequences .
	manualset3
154634	3	408423	13	NULL	NULL	0	NULL	60	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The SVM classification system was further tested on a small class of snRNA-binding proteins with only 60 available sequences .
	manualset3
154635	4	408423	13	NULL	NULL	0	NULL	 sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The SVM classification system was further tested on a small class of snRNA-binding proteins with only 60 available sequences .
	manualset3
154636	1	408424	13	NULL	NULL	0	NULL	Seattle FICSIT/MoveIt study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Seattle FICSIT/MoveIt study is a population-based , randomized , controlled trial comparing the effects of three 6-month exercise interventions ( endurance training , strength training , or combined endurance and strength training ) , and three 3-month endurance training interventions ( stationary cycle , walking , or aerobic movement ) .
	manualset3
154637	2	408424	13	NULL	NULL	0	NULL	trial	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Seattle FICSIT/MoveIt study is a population-based , randomized , controlled trial comparing the effects of three 6-month exercise interventions ( endurance training , strength training , or combined endurance and strength training ) , and three 3-month endurance training interventions ( stationary cycle , walking , or aerobic movement ) .
	manualset3
154638	3	408424	13	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Seattle FICSIT/MoveIt study is a population-based , randomized , controlled trial comparing the effects of three 6-month exercise interventions ( endurance training , strength training , or combined endurance and strength training ) , and three 3-month endurance training interventions ( stationary cycle , walking , or aerobic movement ) .
	manualset3
154639	4	408424	13	NULL	NULL	0	NULL	 three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Seattle FICSIT/MoveIt study is a population-based , randomized , controlled trial comparing the effects of three 6-month exercise interventions ( endurance training , strength training , or combined endurance and strength training ) , and three 3-month endurance training interventions ( stationary cycle , walking , or aerobic movement ) .
	manualset3
154640	5	408424	13	NULL	NULL	0	NULL	6-month	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The Seattle FICSIT/MoveIt study is a population-based , randomized , controlled trial comparing the effects of three 6-month exercise interventions ( endurance training , strength training , or combined endurance and strength training ) , and three 3-month endurance training interventions ( stationary cycle , walking , or aerobic movement ) .
	manualset3
154641	6	408424	13	NULL	NULL	0	NULL	exercise interventions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Seattle FICSIT/MoveIt study is a population-based , randomized , controlled trial comparing the effects of three 6-month exercise interventions ( endurance training , strength training , or combined endurance and strength training ) , and three 3-month endurance training interventions ( stationary cycle , walking , or aerobic movement ) .
	manualset3
154642	7	408424	13	NULL	NULL	0	NULL	endurance training 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Seattle FICSIT/MoveIt study is a population-based , randomized , controlled trial comparing the effects of three 6-month exercise interventions ( endurance training , strength training , or combined endurance and strength training ) , and three 3-month endurance training interventions ( stationary cycle , walking , or aerobic movement ) .
	manualset3
154643	8	408424	13	NULL	NULL	0	NULL	strength training 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Seattle FICSIT/MoveIt study is a population-based , randomized , controlled trial comparing the effects of three 6-month exercise interventions ( endurance training , strength training , or combined endurance and strength training ) , and three 3-month endurance training interventions ( stationary cycle , walking , or aerobic movement ) .
	manualset3
154644	9	408424	13	NULL	NULL	0	NULL	combined endurance and strength training 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Seattle FICSIT/MoveIt study is a population-based , randomized , controlled trial comparing the effects of three 6-month exercise interventions ( endurance training , strength training , or combined endurance and strength training ) , and three 3-month endurance training interventions ( stationary cycle , walking , or aerobic movement ) .
	manualset3
154645	10	408424	13	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Seattle FICSIT/MoveIt study is a population-based , randomized , controlled trial comparing the effects of three 6-month exercise interventions ( endurance training , strength training , or combined endurance and strength training ) , and three 3-month endurance training interventions ( stationary cycle , walking , or aerobic movement ) .
	manualset3
154646	11	408424	13	NULL	NULL	0	NULL	3-month	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The Seattle FICSIT/MoveIt study is a population-based , randomized , controlled trial comparing the effects of three 6-month exercise interventions ( endurance training , strength training , or combined endurance and strength training ) , and three 3-month endurance training interventions ( stationary cycle , walking , or aerobic movement ) .
	manualset3
154647	12	408424	13	NULL	NULL	0	NULL	endurance training interventions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Seattle FICSIT/MoveIt study is a population-based , randomized , controlled trial comparing the effects of three 6-month exercise interventions ( endurance training , strength training , or combined endurance and strength training ) , and three 3-month endurance training interventions ( stationary cycle , walking , or aerobic movement ) .
	manualset3
154648	13	408424	13	NULL	NULL	0	NULL	stationary cycle	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Seattle FICSIT/MoveIt study is a population-based , randomized , controlled trial comparing the effects of three 6-month exercise interventions ( endurance training , strength training , or combined endurance and strength training ) , and three 3-month endurance training interventions ( stationary cycle , walking , or aerobic movement ) .
	manualset3
154649	14	408424	13	NULL	NULL	0	NULL	aerobic movement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Seattle FICSIT/MoveIt study is a population-based , randomized , controlled trial comparing the effects of three 6-month exercise interventions ( endurance training , strength training , or combined endurance and strength training ) , and three 3-month endurance training interventions ( stationary cycle , walking , or aerobic movement ) .
	manualset3
154650	1	408425	13	NULL	NULL	0	NULL	Second National Health and Nutrition Examination Survey 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Second National Health and Nutrition Examination Survey found low iron and zinc intakes and low serum ferritin in many premenopausal women .
	manualset3
154651	2	408425	13	NULL	NULL	0	NULL	 iron 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The Second National Health and Nutrition Examination Survey found low iron and zinc intakes and low serum ferritin in many premenopausal women .
	manualset3
154652	3	408425	13	NULL	NULL	0	NULL	zinc 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The Second National Health and Nutrition Examination Survey found low iron and zinc intakes and low serum ferritin in many premenopausal women .
	manualset3
154653	4	408425	13	NULL	NULL	0	NULL	intakes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Second National Health and Nutrition Examination Survey found low iron and zinc intakes and low serum ferritin in many premenopausal women .
	manualset3
154654	5	408425	13	NULL	NULL	0	NULL	serum ferritin	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Second National Health and Nutrition Examination Survey found low iron and zinc intakes and low serum ferritin in many premenopausal women .
	manualset3
154655	6	408425	13	NULL	NULL	0	NULL	premenopausal women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The Second National Health and Nutrition Examination Survey found low iron and zinc intakes and low serum ferritin in many premenopausal women .
	manualset3
154656	1	408426	13	NULL	NULL	0	NULL	Seroprevalence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Seroprevalence was more among persons of higher age group .
	manualset3
154657	2	408426	13	NULL	NULL	0	NULL	persons	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The Seroprevalence was more among persons of higher age group .
	manualset3
154658	3	408426	13	NULL	NULL	0	NULL	higher age group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The Seroprevalence was more among persons of higher age group .
	manualset3
154659	1	408427	13	NULL	NULL	0	NULL	She2p/mRNA complex	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The She2p/mRNA complex subsequently associates with the myosin motor protein , Myo4p , through an adapter , She3p .
	manualset3
154660	2	408427	13	NULL	NULL	0	NULL	myosin motor protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The She2p/mRNA complex subsequently associates with the myosin motor protein , Myo4p , through an adapter , She3p .
	manualset3
154661	3	408427	13	NULL	NULL	0	NULL	Myo4p	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The She2p/mRNA complex subsequently associates with the myosin motor protein , Myo4p , through an adapter , She3p .
	manualset3
154662	4	408427	13	NULL	NULL	0	NULL	adapter	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The She2p/mRNA complex subsequently associates with the myosin motor protein , Myo4p , through an adapter , She3p .
	manualset3
154663	5	408427	13	NULL	NULL	0	NULL	She3p	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The She2p/mRNA complex subsequently associates with the myosin motor protein , Myo4p , through an adapter , She3p .
	manualset3
154664	1	408428	13	NULL	NULL	0	NULL	Sig proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The Sig proteins are thought to play a role in mediating sperm-egg recognition during the sexual reproduction phase .
	manualset3
154665	2	408428	13	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Sig proteins are thought to play a role in mediating sperm-egg recognition during the sexual reproduction phase .
	manualset3
154666	3	408428	13	NULL	NULL	0	NULL	sperm-egg recognition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Sig proteins are thought to play a role in mediating sperm-egg recognition during the sexual reproduction phase .
	manualset3
154667	4	408428	13	NULL	NULL	0	NULL	sexual reproduction phase	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The Sig proteins are thought to play a role in mediating sperm-egg recognition during the sexual reproduction phase .
	manualset3
154668	1	408429	13	NULL	NULL	0	NULL	ratio	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A relatively constant ratio of bone marrow precursors to B cells of immature phenotype ( CD24highCD10 + CD20lowIgD - ) is maintained from mid-gestation through the eighth decade of life .
	manualset3
154669	2	408429	13	NULL	NULL	0	NULL	bone marrow precursors	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A relatively constant ratio of bone marrow precursors to B cells of immature phenotype ( CD24highCD10 + CD20lowIgD - ) is maintained from mid-gestation through the eighth decade of life .
	manualset3
154670	3	408429	13	NULL	NULL	0	NULL	B cells	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A relatively constant ratio of bone marrow precursors to B cells of immature phenotype ( CD24highCD10 + CD20lowIgD - ) is maintained from mid-gestation through the eighth decade of life .
	manualset3
154671	4	408429	13	NULL	NULL	NULL	NULL	immature phenotype ( CD24highCD10 + CD20lowIgD - ) 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A relatively constant ratio of bone marrow precursors to B cells of immature phenotype ( CD24highCD10 + CD20lowIgD - ) is maintained from mid-gestation through the eighth decade of life .
	manualset3
154672	5	408429	13	NULL	NULL	0	NULL	mid-gestation 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A relatively constant ratio of bone marrow precursors to B cells of immature phenotype ( CD24highCD10 + CD20lowIgD - ) is maintained from mid-gestation through the eighth decade of life .
	manualset3
154673	6	408429	13	NULL	NULL	0	NULL	eighth decade	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A relatively constant ratio of bone marrow precursors to B cells of immature phenotype ( CD24highCD10 + CD20lowIgD - ) is maintained from mid-gestation through the eighth decade of life .
	manualset3
154674	7	408429	13	NULL	NULL	0	NULL	life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A relatively constant ratio of bone marrow precursors to B cells of immature phenotype ( CD24highCD10 + CD20lowIgD - ) is maintained from mid-gestation through the eighth decade of life .
	manualset3
154675	1	408430	13	NULL	NULL	0	NULL	Suicide Opinion Questionnaire ( SOQ )	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Suicide Opinion Questionnaire ( SOQ ) was administered to two samples of medical school students , from Japan ( n = 80 males and 20 females ) and the United States ( n = 80 males and 20 females ) .
	manualset3
154676	2	408430	13	NULL	NULL	0	NULL	two samples 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The Suicide Opinion Questionnaire ( SOQ ) was administered to two samples of medical school students , from Japan ( n = 80 males and 20 females ) and the United States ( n = 80 males and 20 females ) .
	manualset3
154677	3	408430	13	NULL	NULL	0	NULL	medical school students	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The Suicide Opinion Questionnaire ( SOQ ) was administered to two samples of medical school students , from Japan ( n = 80 males and 20 females ) and the United States ( n = 80 males and 20 females ) .
	manualset3
154678	4	408430	13	NULL	NULL	0	NULL	Japan	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The Suicide Opinion Questionnaire ( SOQ ) was administered to two samples of medical school students , from Japan ( n = 80 males and 20 females ) and the United States ( n = 80 males and 20 females ) .
	manualset3
154679	5	408430	13	NULL	NULL	0	NULL	n = 80 males and 20 females	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Suicide Opinion Questionnaire ( SOQ ) was administered to two samples of medical school students , from Japan ( n = 80 males and 20 females ) and the United States ( n = 80 males and 20 females ) .
	manualset3
154680	6	408430	13	NULL	NULL	0	NULL	United States 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The Suicide Opinion Questionnaire ( SOQ ) was administered to two samples of medical school students , from Japan ( n = 80 males and 20 females ) and the United States ( n = 80 males and 20 females ) .
	manualset3
154681	7	408430	13	NULL	NULL	0	NULL	n = 80 males and 20 females	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Suicide Opinion Questionnaire ( SOQ ) was administered to two samples of medical school students , from Japan ( n = 80 males and 20 females ) and the United States ( n = 80 males and 20 females ) .
	manualset3
154682	1	408431	13	NULL	NULL	0	NULL	Sulfur Oxygenase Reductase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The Sulfur Oxygenase Reductase from the Mesophilic Bacterium Halothiobacillus neapolitanus Is a Highly Active Thermozyme .
	manualset3
154683	2	408431	13	NULL	NULL	0	NULL	Mesophilic Bacterium Halothiobacillus neapolitanus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The Sulfur Oxygenase Reductase from the Mesophilic Bacterium Halothiobacillus neapolitanus Is a Highly Active Thermozyme .
	manualset3
154684	3	408431	13	NULL	NULL	0	NULL	Thermozyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The Sulfur Oxygenase Reductase from the Mesophilic Bacterium Halothiobacillus neapolitanus Is a Highly Active Thermozyme .
	manualset3
154685	1	408432	13	NULL	NULL	0	NULL	Supreme Court	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The Supreme Court decided an issue that is critical to consumer health and safety last year .
	manualset3
154686	2	408432	13	NULL	NULL	0	NULL	issue	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Supreme Court decided an issue that is critical to consumer health and safety last year .
	manualset3
154687	3	408432	13	NULL	NULL	0	NULL	consumer health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Supreme Court decided an issue that is critical to consumer health and safety last year .
	manualset3
154688	4	408432	13	NULL	NULL	0	NULL	last year	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The Supreme Court decided an issue that is critical to consumer health and safety last year .
	manualset3
154689	1	408433	13	NULL	NULL	0	NULL	T-cell immunoglobulin and mucin domain 3 ( TIM-3 )	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The T-cell immunoglobulin and mucin domain 3 ( TIM-3 ) has been shown to be associated with susceptibility to rheumatoid arthritis ( RA ) .
	manualset3
154690	2	408433	13	NULL	NULL	0	NULL	susceptibility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The T-cell immunoglobulin and mucin domain 3 ( TIM-3 ) has been shown to be associated with susceptibility to rheumatoid arthritis ( RA ) .
	manualset3
154691	3	408433	13	NULL	NULL	0	NULL	rheumatoid arthritis ( RA ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The T-cell immunoglobulin and mucin domain 3 ( TIM-3 ) has been shown to be associated with susceptibility to rheumatoid arthritis ( RA ) .
	manualset3
154692	1	408434	13	NULL	NULL	0	NULL	T cells	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The T cells from both breeds recognized most of the mycobacterial antigens at lower and comparable frequencies .
	manualset3
154693	2	408434	13	NULL	NULL	0	NULL	breeds 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The T cells from both breeds recognized most of the mycobacterial antigens at lower and comparable frequencies .
	manualset3
154694	3	408434	13	NULL	NULL	0	NULL	mycobacterial antigens	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The T cells from both breeds recognized most of the mycobacterial antigens at lower and comparable frequencies .
	manualset3
154695	4	408434	13	NULL	NULL	0	NULL	frequencies	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The T cells from both breeds recognized most of the mycobacterial antigens at lower and comparable frequencies .
	manualset3
154696	1	408435	13	NULL	NULL	0	NULL	T178S substitution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The T178S , T178V , V203A , V292A , V292S , and V292T substitutions significantly alter the steady state and transient kinetics of the enzyme .
	manualset3
154697	2	408435	13	NULL	NULL	0	NULL	T178V substitution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The T178S , T178V , V203A , V292A , V292S , and V292T substitutions significantly alter the steady state and transient kinetics of the enzyme .
	manualset3
154698	3	408435	13	NULL	NULL	0	NULL	V203A substitution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The T178S , T178V , V203A , V292A , V292S , and V292T substitutions significantly alter the steady state and transient kinetics of the enzyme .
	manualset3
154699	4	408435	13	NULL	NULL	0	NULL	V292A substitution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The T178S , T178V , V203A , V292A , V292S , and V292T substitutions significantly alter the steady state and transient kinetics of the enzyme .
	manualset3
154700	5	408435	13	NULL	NULL	0	NULL	V292S substitution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The T178S , T178V , V203A , V292A , V292S , and V292T substitutions significantly alter the steady state and transient kinetics of the enzyme .
	manualset3
154701	6	408435	13	NULL	NULL	0	NULL	V292T substitution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The T178S , T178V , V203A , V292A , V292S , and V292T substitutions significantly alter the steady state and transient kinetics of the enzyme .
	manualset3
154702	7	408435	13	NULL	NULL	0	NULL	steady state 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The T178S , T178V , V203A , V292A , V292S , and V292T substitutions significantly alter the steady state and transient kinetics of the enzyme .
	manualset3
154703	8	408435	13	NULL	NULL	0	NULL	transient kinetics	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The T178S , T178V , V203A , V292A , V292S , and V292T substitutions significantly alter the steady state and transient kinetics of the enzyme .
	manualset3
154704	9	408435	13	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The T178S , T178V , V203A , V292A , V292S , and V292T substitutions significantly alter the steady state and transient kinetics of the enzyme .
	manualset3
154705	1	408436	13	NULL	NULL	0	NULL	level	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A relatively low level of luciferase activity was supported by vector p907 .
	manualset3
154706	2	408436	13	NULL	NULL	0	NULL	luciferase activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A relatively low level of luciferase activity was supported by vector p907 .
	manualset3
154707	3	408436	13	NULL	NULL	0	NULL	vector p907	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A relatively low level of luciferase activity was supported by vector p907 .
	manualset3
154708	1	408437	13	NULL	NULL	0	NULL	T3 dissociation constants	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The T3 dissociation constants were 3.5 , 35 and 115 nM and the number of sites was respectively 0.9 , 20 and 36 X 10 ( 6 ) sites/cell .
	manualset3
154709	2	408437	13	NULL	NULL	0	NULL	3.5 nM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The T3 dissociation constants were 3.5 , 35 and 115 nM and the number of sites was respectively 0.9 , 20 and 36 X 10 ( 6 ) sites/cell .
	manualset3
154710	3	408437	13	NULL	NULL	0	NULL	35 nM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The T3 dissociation constants were 3.5 , 35 and 115 nM and the number of sites was respectively 0.9 , 20 and 36 X 10 ( 6 ) sites/cell .
	manualset3
154711	4	408437	13	NULL	NULL	0	NULL	115 nM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The T3 dissociation constants were 3.5 , 35 and 115 nM and the number of sites was respectively 0.9 , 20 and 36 X 10 ( 6 ) sites/cell .
	manualset3
154712	5	408437	13	NULL	NULL	0	NULL	number of sites 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The T3 dissociation constants were 3.5 , 35 and 115 nM and the number of sites was respectively 0.9 , 20 and 36 X 10 ( 6 ) sites/cell .
	manualset3
154713	6	408437	13	NULL	NULL	NULL	NULL	0.9 X 10 ( 6 ) sites/cell	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The T3 dissociation constants were 3.5 , 35 and 115 nM and the number of sites was respectively 0.9 , 20 and 36 X 10 ( 6 ) sites/cell .
	manualset3
154714	7	408437	13	NULL	NULL	NULL	NULL	20 X 10 ( 6 ) sites/cell	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The T3 dissociation constants were 3.5 , 35 and 115 nM and the number of sites was respectively 0.9 , 20 and 36 X 10 ( 6 ) sites/cell .
	manualset3
154715	8	408437	13	NULL	NULL	0	NULL	36 X 10 ( 6 ) sites/cell	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The T3 dissociation constants were 3.5 , 35 and 115 nM and the number of sites was respectively 0.9 , 20 and 36 X 10 ( 6 ) sites/cell .
	manualset3
154716	1	408438	13	NULL	NULL	0	NULL	TASK subfamily of K2P channels	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The TASK subfamily of K2P channels are inhibited following activation of the G protein Galpha ( q ) .
	manualset3
154717	2	408438	13	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The TASK subfamily of K2P channels are inhibited following activation of the G protein Galpha ( q ) .
	manualset3
154718	3	408438	13	NULL	NULL	0	NULL	G protein Galpha ( q ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The TASK subfamily of K2P channels are inhibited following activation of the G protein Galpha ( q ) .
	manualset3
154719	1	408439	13	NULL	NULL	0	NULL	TCL	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The TCL were stained for CD3 , CD4 , CD8 , TCR alpha beta and gamma delta expression by indirect immunofluorescence , and their proliferative responses to mitogens and gluten fraction III ( a peptic-tryptic digest of gluten ) investigated .
	manualset3
154720	2	408439	13	NULL	NULL	0	NULL	CD3 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The TCL were stained for CD3 , CD4 , CD8 , TCR alpha beta and gamma delta expression by indirect immunofluorescence , and their proliferative responses to mitogens and gluten fraction III ( a peptic-tryptic digest of gluten ) investigated .
	manualset3
154721	3	408439	13	NULL	NULL	0	NULL	CD4 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The TCL were stained for CD3 , CD4 , CD8 , TCR alpha beta and gamma delta expression by indirect immunofluorescence , and their proliferative responses to mitogens and gluten fraction III ( a peptic-tryptic digest of gluten ) investigated .
	manualset3
154722	4	408439	13	NULL	NULL	0	NULL	CD8 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The TCL were stained for CD3 , CD4 , CD8 , TCR alpha beta and gamma delta expression by indirect immunofluorescence , and their proliferative responses to mitogens and gluten fraction III ( a peptic-tryptic digest of gluten ) investigated .
	manualset3
154723	5	408439	13	NULL	NULL	0	NULL	TCR alpha expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The TCL were stained for CD3 , CD4 , CD8 , TCR alpha beta and gamma delta expression by indirect immunofluorescence , and their proliferative responses to mitogens and gluten fraction III ( a peptic-tryptic digest of gluten ) investigated .
	manualset3
154724	6	408439	13	NULL	NULL	0	NULL	TCR beta expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The TCL were stained for CD3 , CD4 , CD8 , TCR alpha beta and gamma delta expression by indirect immunofluorescence , and their proliferative responses to mitogens and gluten fraction III ( a peptic-tryptic digest of gluten ) investigated .
	manualset3
154725	7	408439	13	NULL	NULL	0	NULL	TCR gamma expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The TCL were stained for CD3 , CD4 , CD8 , TCR alpha beta and gamma delta expression by indirect immunofluorescence , and their proliferative responses to mitogens and gluten fraction III ( a peptic-tryptic digest of gluten ) investigated .
	manualset3
154726	8	408439	13	NULL	NULL	0	NULL	TCR delta expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The TCL were stained for CD3 , CD4 , CD8 , TCR alpha beta and gamma delta expression by indirect immunofluorescence , and their proliferative responses to mitogens and gluten fraction III ( a peptic-tryptic digest of gluten ) investigated .
	manualset3
154727	9	408439	13	NULL	NULL	0	NULL	immunofluorescence 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The TCL were stained for CD3 , CD4 , CD8 , TCR alpha beta and gamma delta expression by indirect immunofluorescence , and their proliferative responses to mitogens and gluten fraction III ( a peptic-tryptic digest of gluten ) investigated .
	manualset3
154728	10	408439	13	NULL	NULL	0	NULL	proliferative responses	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The TCL were stained for CD3 , CD4 , CD8 , TCR alpha beta and gamma delta expression by indirect immunofluorescence , and their proliferative responses to mitogens and gluten fraction III ( a peptic-tryptic digest of gluten ) investigated .
	manualset3
154729	11	408439	13	NULL	NULL	0	NULL	mitogens 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The TCL were stained for CD3 , CD4 , CD8 , TCR alpha beta and gamma delta expression by indirect immunofluorescence , and their proliferative responses to mitogens and gluten fraction III ( a peptic-tryptic digest of gluten ) investigated .
	manualset3
154730	12	408439	13	NULL	NULL	0	NULL	gluten fraction III 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The TCL were stained for CD3 , CD4 , CD8 , TCR alpha beta and gamma delta expression by indirect immunofluorescence , and their proliferative responses to mitogens and gluten fraction III ( a peptic-tryptic digest of gluten ) investigated .
	manualset3
154731	13	408439	13	NULL	NULL	0	NULL	peptic-tryptic digest of gluten	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The TCL were stained for CD3 , CD4 , CD8 , TCR alpha beta and gamma delta expression by indirect immunofluorescence , and their proliferative responses to mitogens and gluten fraction III ( a peptic-tryptic digest of gluten ) investigated .
	manualset3
154732	1	408440	13	NULL	NULL	0	NULL	cell shrinkage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The TEA-induced cell shrinkage was inhibited by ouabain , suggesting that TEA increases Na + - K + pump activity .
	manualset3
154733	2	408440	13	NULL	NULL	0	NULL	ouabain	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The TEA-induced cell shrinkage was inhibited by ouabain , suggesting that TEA increases Na + - K + pump activity .
	manualset3
154734	3	408440	13	NULL	NULL	0	NULL	TEA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The TEA-induced cell shrinkage was inhibited by ouabain , suggesting that TEA increases Na + - K + pump activity .
	manualset3
154735	4	408440	13	NULL	NULL	0	NULL	increases	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The TEA-induced cell shrinkage was inhibited by ouabain , suggesting that TEA increases Na + - K + pump activity .
	manualset3
154736	5	408440	13	NULL	NULL	0	NULL	Na + - K + pump activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The TEA-induced cell shrinkage was inhibited by ouabain , suggesting that TEA increases Na + - K + pump activity .
	manualset3
154737	1	408441	13	NULL	NULL	0	NULL	TEC antigens 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The TEC antigens have been identified on mouse preimplantation embryos , and their expression is specific to particular developmental stages .
	manualset3
154738	2	408441	13	NULL	NULL	0	NULL	mouse preimplantation embryos	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The TEC antigens have been identified on mouse preimplantation embryos , and their expression is specific to particular developmental stages .
	manualset3
154739	3	408441	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The TEC antigens have been identified on mouse preimplantation embryos , and their expression is specific to particular developmental stages .
	manualset3
154740	4	408441	13	NULL	NULL	0	NULL	developmental stages	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The TEC antigens have been identified on mouse preimplantation embryos , and their expression is specific to particular developmental stages .
	manualset3
154741	1	408442	13	NULL	NULL	0	NULL	TERT ( telomerase reverse transcriptase ) subunit of telomerase 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The TERT ( telomerase reverse transcriptase ) subunit of telomerase is an intensively studied macromolecule due to its key importance in maintaining genome integrity and role in cellular aging and cancer .
	manualset3
154742	2	408442	13	NULL	NULL	0	NULL	macromolecule	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The TERT ( telomerase reverse transcriptase ) subunit of telomerase is an intensively studied macromolecule due to its key importance in maintaining genome integrity and role in cellular aging and cancer .
	manualset3
154743	3	408442	13	NULL	NULL	0	NULL	importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The TERT ( telomerase reverse transcriptase ) subunit of telomerase is an intensively studied macromolecule due to its key importance in maintaining genome integrity and role in cellular aging and cancer .
	manualset3
154744	4	408442	13	NULL	NULL	0	NULL	genome integrity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The TERT ( telomerase reverse transcriptase ) subunit of telomerase is an intensively studied macromolecule due to its key importance in maintaining genome integrity and role in cellular aging and cancer .
	manualset3
154745	5	408442	13	NULL	NULL	0	NULL	role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The TERT ( telomerase reverse transcriptase ) subunit of telomerase is an intensively studied macromolecule due to its key importance in maintaining genome integrity and role in cellular aging and cancer .
	manualset3
154746	6	408442	13	NULL	NULL	0	NULL	cellular aging	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The TERT ( telomerase reverse transcriptase ) subunit of telomerase is an intensively studied macromolecule due to its key importance in maintaining genome integrity and role in cellular aging and cancer .
	manualset3
154747	7	408442	13	NULL	NULL	0	NULL	cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The TERT ( telomerase reverse transcriptase ) subunit of telomerase is an intensively studied macromolecule due to its key importance in maintaining genome integrity and role in cellular aging and cancer .
	manualset3
154748	1	408443	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The TFP-stimulated increase of the Egr-1 protein was preferentially inhibited by the MEK-specific inhibitor PD98059 .
	manualset3
154749	2	408443	13	NULL	NULL	0	NULL	Egr-1 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The TFP-stimulated increase of the Egr-1 protein was preferentially inhibited by the MEK-specific inhibitor PD98059 .
	manualset3
154750	3	408443	13	NULL	NULL	0	NULL	MEK-specific inhibitor PD98059	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The TFP-stimulated increase of the Egr-1 protein was preferentially inhibited by the MEK-specific inhibitor PD98059 .
	manualset3
154751	1	408444	13	NULL	NULL	0	NULL	TG profiles	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The TG profiles indicated that BNCP , BNNP and MNCuP are thermally stable up to the temperature of 260-278 degrees C unlike MNZnP ( 150 degrees C ) .
	manualset3
154752	2	408444	13	NULL	NULL	0	NULL	BNCP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The TG profiles indicated that BNCP , BNNP and MNCuP are thermally stable up to the temperature of 260-278 degrees C unlike MNZnP ( 150 degrees C ) .
	manualset3
154753	3	408444	13	NULL	NULL	0	NULL	BNNP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The TG profiles indicated that BNCP , BNNP and MNCuP are thermally stable up to the temperature of 260-278 degrees C unlike MNZnP ( 150 degrees C ) .
	manualset3
154754	4	408444	13	NULL	NULL	0	NULL	MNCuP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The TG profiles indicated that BNCP , BNNP and MNCuP are thermally stable up to the temperature of 260-278 degrees C unlike MNZnP ( 150 degrees C ) .
	manualset3
154755	5	408444	13	NULL	NULL	0	NULL	temperature	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The TG profiles indicated that BNCP , BNNP and MNCuP are thermally stable up to the temperature of 260-278 degrees C unlike MNZnP ( 150 degrees C ) .
	manualset3
154756	6	408444	13	NULL	NULL	0	NULL	260-278 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The TG profiles indicated that BNCP , BNNP and MNCuP are thermally stable up to the temperature of 260-278 degrees C unlike MNZnP ( 150 degrees C ) .
	manualset3
154757	7	408444	13	NULL	NULL	0	NULL	MNZnP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The TG profiles indicated that BNCP , BNNP and MNCuP are thermally stable up to the temperature of 260-278 degrees C unlike MNZnP ( 150 degrees C ) .
	manualset3
154758	8	408444	13	NULL	NULL	0	NULL	150 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The TG profiles indicated that BNCP , BNNP and MNCuP are thermally stable up to the temperature of 260-278 degrees C unlike MNZnP ( 150 degrees C ) .
	manualset3
154759	1	408445	13	NULL	NULL	0	NULL	TGF-beta 2-induced increment 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The TGF-beta 2-induced increment of PAF receptor mRNA was at least partly due to an increase in transcriptional rate as demonstrated by nuclear run-off experiments .
	manualset3
154760	2	408445	13	NULL	NULL	0	NULL	PAF receptor mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The TGF-beta 2-induced increment of PAF receptor mRNA was at least partly due to an increase in transcriptional rate as demonstrated by nuclear run-off experiments .
	manualset3
154761	3	408445	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The TGF-beta 2-induced increment of PAF receptor mRNA was at least partly due to an increase in transcriptional rate as demonstrated by nuclear run-off experiments .
	manualset3
154762	4	408445	13	NULL	NULL	0	NULL	transcriptional rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The TGF-beta 2-induced increment of PAF receptor mRNA was at least partly due to an increase in transcriptional rate as demonstrated by nuclear run-off experiments .
	manualset3
154763	5	408445	13	NULL	NULL	0	NULL	nuclear run-off experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The TGF-beta 2-induced increment of PAF receptor mRNA was at least partly due to an increase in transcriptional rate as demonstrated by nuclear run-off experiments .
	manualset3
154764	1	408446	13	NULL	NULL	0	NULL	TM regions	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The TM regions of two mutant receptors were either extended ( designated i626-3 ) or shortened ( designated d625 .3 ) by three hydrophobic amino acid residues .
	manualset3
154765	2	408446	13	NULL	NULL	0	NULL	two mutant receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The TM regions of two mutant receptors were either extended ( designated i626-3 ) or shortened ( designated d625 .3 ) by three hydrophobic amino acid residues .
	manualset3
154766	3	408446	13	NULL	NULL	0	NULL	i626-3 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The TM regions of two mutant receptors were either extended ( designated i626-3 ) or shortened ( designated d625 .3 ) by three hydrophobic amino acid residues .
	manualset3
154767	4	408446	13	NULL	NULL	0	NULL	d625 .3 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The TM regions of two mutant receptors were either extended ( designated i626-3 ) or shortened ( designated d625 .3 ) by three hydrophobic amino acid residues .
	manualset3
154768	5	408446	13	NULL	NULL	0	NULL	three hydrophobic amino acid residues 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The TM regions of two mutant receptors were either extended ( designated i626-3 ) or shortened ( designated d625 .3 ) by three hydrophobic amino acid residues .
	manualset3
154769	1	408447	13	NULL	NULL	0	NULL	TMPG reagent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The TMPG reagent specifically reacted with guanine moiety in DNA at room temperature and provided CL intensities .
	manualset3
154770	2	408447	13	NULL	NULL	0	NULL	guanine moiety	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The TMPG reagent specifically reacted with guanine moiety in DNA at room temperature and provided CL intensities .
	manualset3
154771	3	408447	13	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The TMPG reagent specifically reacted with guanine moiety in DNA at room temperature and provided CL intensities .
	manualset3
154772	4	408447	13	NULL	NULL	0	NULL	room temperature 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The TMPG reagent specifically reacted with guanine moiety in DNA at room temperature and provided CL intensities .
	manualset3
154773	5	408447	13	NULL	NULL	0	NULL	CL intensities	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The TMPG reagent specifically reacted with guanine moiety in DNA at room temperature and provided CL intensities .
	manualset3
154774	1	408448	13	NULL	NULL	0	NULL	TPST activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The TPST activity was also stimulated by two other major prostaglandins of salivary glands , PGF2 alpha and 6-Keto-PGF 1 alpha , however to lesser extent , 22 and 23 % , respectively .
	manualset3
154775	2	408448	13	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The TPST activity was also stimulated by two other major prostaglandins of salivary glands , PGF2 alpha and 6-Keto-PGF 1 alpha , however to lesser extent , 22 and 23 % , respectively .
	manualset3
154776	3	408448	13	NULL	NULL	0	NULL	prostaglandins 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The TPST activity was also stimulated by two other major prostaglandins of salivary glands , PGF2 alpha and 6-Keto-PGF 1 alpha , however to lesser extent , 22 and 23 % , respectively .
	manualset3
154777	4	408448	13	NULL	NULL	0	NULL	salivary glands	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The TPST activity was also stimulated by two other major prostaglandins of salivary glands , PGF2 alpha and 6-Keto-PGF 1 alpha , however to lesser extent , 22 and 23 % , respectively .
	manualset3
154779	5	408448	13	NULL	NULL	0	NULL	PGF2 alpha	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The TPST activity was also stimulated by two other major prostaglandins of salivary glands , PGF2 alpha and 6-Keto-PGF 1 alpha , however to lesser extent , 22 and 23 % , respectively .
	manualset3
154780	6	408448	13	NULL	NULL	0	NULL	6-Keto-PGF 1 alpha	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The TPST activity was also stimulated by two other major prostaglandins of salivary glands , PGF2 alpha and 6-Keto-PGF 1 alpha , however to lesser extent , 22 and 23 % , respectively .
	manualset3
154781	7	408448	13	NULL	NULL	0	NULL	 22 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The TPST activity was also stimulated by two other major prostaglandins of salivary glands , PGF2 alpha and 6-Keto-PGF 1 alpha , however to lesser extent , 22 and 23 % , respectively .
	manualset3
154782	8	408448	13	NULL	NULL	0	NULL	23 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The TPST activity was also stimulated by two other major prostaglandins of salivary glands , PGF2 alpha and 6-Keto-PGF 1 alpha , however to lesser extent , 22 and 23 % , respectively .
	manualset3
154783	1	408449	13	NULL	NULL	0	NULL	TS	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The TS and LSM showed a better homogeneity of the distribution of the spray .
	manualset3
154784	2	408449	13	NULL	NULL	0	NULL	LSM	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The TS and LSM showed a better homogeneity of the distribution of the spray .
	manualset3
154785	3	408449	13	NULL	NULL	0	NULL	homogeneity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The TS and LSM showed a better homogeneity of the distribution of the spray .
	manualset3
154786	4	408449	13	NULL	NULL	0	NULL	distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The TS and LSM showed a better homogeneity of the distribution of the spray .
	manualset3
154787	5	408449	13	NULL	NULL	0	NULL	spray	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The TS and LSM showed a better homogeneity of the distribution of the spray .
	manualset3
154788	1	408450	13	NULL	NULL	0	NULL	TSH-induced effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The TSH-induced effect in each case is inhibited by cycloheximide ; the TSH-induced decrease in SSBP/DNA complex formation requires the presence of insulin or calf serum , exactly as does TSH-induced down-regulation of TSHR RNA levels .
	manualset3
154789	2	408450	13	NULL	NULL	0	NULL	case	NamedEntity 												NULL		0	NULL	NULL	NULL	NULL	NULL	The TSH-induced effect in each case is inhibited by cycloheximide ; the TSH-induced decrease in SSBP/DNA complex formation requires the presence of insulin or calf serum , exactly as does TSH-induced down-regulation of TSHR RNA levels .
	manualset3
154790	3	408450	13	NULL	NULL	0	NULL	cycloheximide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The TSH-induced effect in each case is inhibited by cycloheximide ; the TSH-induced decrease in SSBP/DNA complex formation requires the presence of insulin or calf serum , exactly as does TSH-induced down-regulation of TSHR RNA levels .
	manualset3
154791	4	408450	13	NULL	NULL	0	NULL	TSH-induced decrease	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The TSH-induced effect in each case is inhibited by cycloheximide ; the TSH-induced decrease in SSBP/DNA complex formation requires the presence of insulin or calf serum , exactly as does TSH-induced down-regulation of TSHR RNA levels .
	manualset3
154792	5	408450	13	NULL	NULL	0	NULL	SSBP/DNA complex formation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The TSH-induced effect in each case is inhibited by cycloheximide ; the TSH-induced decrease in SSBP/DNA complex formation requires the presence of insulin or calf serum , exactly as does TSH-induced down-regulation of TSHR RNA levels .
	manualset3
154793	6	408450	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The TSH-induced effect in each case is inhibited by cycloheximide ; the TSH-induced decrease in SSBP/DNA complex formation requires the presence of insulin or calf serum , exactly as does TSH-induced down-regulation of TSHR RNA levels .
	manualset3
154794	7	408450	13	NULL	NULL	0	NULL	insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The TSH-induced effect in each case is inhibited by cycloheximide ; the TSH-induced decrease in SSBP/DNA complex formation requires the presence of insulin or calf serum , exactly as does TSH-induced down-regulation of TSHR RNA levels .
	manualset3
154795	8	408450	13	NULL	NULL	0	NULL	calf serum	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The TSH-induced effect in each case is inhibited by cycloheximide ; the TSH-induced decrease in SSBP/DNA complex formation requires the presence of insulin or calf serum , exactly as does TSH-induced down-regulation of TSHR RNA levels .
	manualset3
154796	9	408450	13	NULL	NULL	0	NULL	TSH-induced down-regulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The TSH-induced effect in each case is inhibited by cycloheximide ; the TSH-induced decrease in SSBP/DNA complex formation requires the presence of insulin or calf serum , exactly as does TSH-induced down-regulation of TSHR RNA levels .
	manualset3
154797	10	408450	13	NULL	NULL	0	NULL	TSHR RNA levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The TSH-induced effect in each case is inhibited by cycloheximide ; the TSH-induced decrease in SSBP/DNA complex formation requires the presence of insulin or calf serum , exactly as does TSH-induced down-regulation of TSHR RNA levels .
	manualset3
154801	1	408451	13	NULL	NULL	0	NULL	TSH response 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The TSH response to TRH , PRL responses to TRH and haloperidol , and LH responses to LHRH were less in the 8 days posttransplants than in the groups studied at 4 days posttransplantation .
	manualset3
154802	2	408451	13	NULL	NULL	0	NULL	 TRH response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The TSH response to TRH , PRL responses to TRH and haloperidol , and LH responses to LHRH were less in the 8 days posttransplants than in the groups studied at 4 days posttransplantation .
	manualset3
154803	3	408451	13	NULL	NULL	0	NULL	PRL response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The TSH response to TRH , PRL responses to TRH and haloperidol , and LH responses to LHRH were less in the 8 days posttransplants than in the groups studied at 4 days posttransplantation .
	manualset3
154804	4	408451	13	NULL	NULL	0	NULL	TRH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The TSH response to TRH , PRL responses to TRH and haloperidol , and LH responses to LHRH were less in the 8 days posttransplants than in the groups studied at 4 days posttransplantation .
	manualset3
154805	5	408451	13	NULL	NULL	0	NULL	haloperidol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The TSH response to TRH , PRL responses to TRH and haloperidol , and LH responses to LHRH were less in the 8 days posttransplants than in the groups studied at 4 days posttransplantation .
	manualset3
154806	6	408451	13	NULL	NULL	0	NULL	LH responses	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The TSH response to TRH , PRL responses to TRH and haloperidol , and LH responses to LHRH were less in the 8 days posttransplants than in the groups studied at 4 days posttransplantation .
	manualset3
154807	7	408451	13	NULL	NULL	0	NULL	LHRH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The TSH response to TRH , PRL responses to TRH and haloperidol , and LH responses to LHRH were less in the 8 days posttransplants than in the groups studied at 4 days posttransplantation .
	manualset3
154808	8	408451	13	NULL	NULL	0	NULL	8 days 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The TSH response to TRH , PRL responses to TRH and haloperidol , and LH responses to LHRH were less in the 8 days posttransplants than in the groups studied at 4 days posttransplantation .
	manualset3
154809	9	408451	13	NULL	NULL	0	NULL	posttransplants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The TSH response to TRH , PRL responses to TRH and haloperidol , and LH responses to LHRH were less in the 8 days posttransplants than in the groups studied at 4 days posttransplantation .
	manualset3
154810	10	408451	13	NULL	NULL	0	NULL	groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The TSH response to TRH , PRL responses to TRH and haloperidol , and LH responses to LHRH were less in the 8 days posttransplants than in the groups studied at 4 days posttransplantation .
	manualset3
154812	11	408451	13	NULL	NULL	0	NULL	4 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The TSH response to TRH , PRL responses to TRH and haloperidol , and LH responses to LHRH were less in the 8 days posttransplants than in the groups studied at 4 days posttransplantation .
	manualset3
154813	12	408451	13	NULL	NULL	0	NULL	posttransplantation	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The TSH response to TRH , PRL responses to TRH and haloperidol , and LH responses to LHRH were less in the 8 days posttransplants than in the groups studied at 4 days posttransplantation .
	manualset3
154814	1	408452	13	NULL	NULL	0	NULL	TgPhIL1 knockout parasites	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The TgPhIL1 knockout parasites have a distinctly different morphology than wild-type parasites , and normal shape is restored in the knockout background after complementation with the wild-type allele .
	manualset3
154816	2	408452	13	NULL	NULL	0	NULL	morphology	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The TgPhIL1 knockout parasites have a distinctly different morphology than wild-type parasites , and normal shape is restored in the knockout background after complementation with the wild-type allele .
	manualset3
154817	3	408452	13	NULL	NULL	0	NULL	wild-type parasites	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The TgPhIL1 knockout parasites have a distinctly different morphology than wild-type parasites , and normal shape is restored in the knockout background after complementation with the wild-type allele .
	manualset3
154818	4	408452	13	NULL	NULL	0	NULL	shape	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The TgPhIL1 knockout parasites have a distinctly different morphology than wild-type parasites , and normal shape is restored in the knockout background after complementation with the wild-type allele .
	manualset3
154819	5	408452	13	NULL	NULL	0	NULL	background	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The TgPhIL1 knockout parasites have a distinctly different morphology than wild-type parasites , and normal shape is restored in the knockout background after complementation with the wild-type allele .
	manualset3
154820	6	408452	13	NULL	NULL	0	NULL	complementation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The TgPhIL1 knockout parasites have a distinctly different morphology than wild-type parasites , and normal shape is restored in the knockout background after complementation with the wild-type allele .
	manualset3
154821	7	408452	13	NULL	NULL	0	NULL	wild-type allele	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The TgPhIL1 knockout parasites have a distinctly different morphology than wild-type parasites , and normal shape is restored in the knockout background after complementation with the wild-type allele .
	manualset3
154822	1	408453	13	NULL	NULL	0	NULL	TiF4	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The TiF4 treated surfaces , however , do show a statistically significant reduction in the acid solubility of the enamel .
	manualset3
154823	2	408453	13	NULL	NULL	0	NULL	surfaces	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The TiF4 treated surfaces , however , do show a statistically significant reduction in the acid solubility of the enamel .
	manualset3
154824	3	408453	13	NULL	NULL	0	NULL	reduction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The TiF4 treated surfaces , however , do show a statistically significant reduction in the acid solubility of the enamel .
	manualset3
154825	4	408453	13	NULL	NULL	0	NULL	acid solubility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The TiF4 treated surfaces , however , do show a statistically significant reduction in the acid solubility of the enamel .
	manualset3
154826	5	408453	13	NULL	NULL	0	NULL	enamel 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The TiF4 treated surfaces , however , do show a statistically significant reduction in the acid solubility of the enamel .
	manualset3
154827	1	408454	13	NULL	NULL	0	NULL	Tpp2 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The Tpp2 gene is highlighted because it encodes a serine-type endopeptidase functionally similar to the Tssp enzyme .
	manualset3
154828	2	408454	13	NULL	NULL	0	NULL	serine-type endopeptidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The Tpp2 gene is highlighted because it encodes a serine-type endopeptidase functionally similar to the Tssp enzyme .
	manualset3
154829	3	408454	13	NULL	NULL	0	NULL	Tssp enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The Tpp2 gene is highlighted because it encodes a serine-type endopeptidase functionally similar to the Tssp enzyme .
	manualset3
154830	1	408455	13	NULL	NULL	0	NULL	Trolox equivalent antioxidant capacity ( TEAC ) assay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Trolox equivalent antioxidant capacity ( TEAC ) assay was used to provide a ranking order of antioxidant activity .
	manualset3
154831	2	408455	13	NULL	NULL	0	NULL	order	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Trolox equivalent antioxidant capacity ( TEAC ) assay was used to provide a ranking order of antioxidant activity .
	manualset3
154832	3	408455	13	NULL	NULL	0	NULL	antioxidant activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Trolox equivalent antioxidant capacity ( TEAC ) assay was used to provide a ranking order of antioxidant activity .
	manualset3
154833	1	408456	13	NULL	NULL	0	NULL	UCLA experience	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The UCLA experience has been built on the classical techniques of Starzl , yet has forged innovations such as split liver transplantation and use of extended criteria donor organs .
	manualset3
154834	2	408456	13	NULL	NULL	0	NULL	classical techniques	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The UCLA experience has been built on the classical techniques of Starzl , yet has forged innovations such as split liver transplantation and use of extended criteria donor organs .
	manualset3
154835	3	408456	13	NULL	NULL	0	NULL	Starzl	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The UCLA experience has been built on the classical techniques of Starzl , yet has forged innovations such as split liver transplantation and use of extended criteria donor organs .
	manualset3
154836	4	408456	13	NULL	NULL	0	NULL	innovations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The UCLA experience has been built on the classical techniques of Starzl , yet has forged innovations such as split liver transplantation and use of extended criteria donor organs .
	manualset3
154837	5	408456	13	NULL	NULL	0	NULL	split liver transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The UCLA experience has been built on the classical techniques of Starzl , yet has forged innovations such as split liver transplantation and use of extended criteria donor organs .
	manualset3
154838	6	408456	13	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The UCLA experience has been built on the classical techniques of Starzl , yet has forged innovations such as split liver transplantation and use of extended criteria donor organs .
	manualset3
154839	7	408456	13	NULL	NULL	0	NULL	donor organs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The UCLA experience has been built on the classical techniques of Starzl , yet has forged innovations such as split liver transplantation and use of extended criteria donor organs .
	manualset3
154840	1	408457	13	NULL	NULL	0	NULL	US Preventive Services Task Force	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The US Preventive Services Task Force recommends brief interventions for reducing alcohol misuse by adults , including pregnant women .
	manualset3
154841	2	408457	13	NULL	NULL	0	NULL	interventions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The US Preventive Services Task Force recommends brief interventions for reducing alcohol misuse by adults , including pregnant women .
	manualset3
154842	3	408457	13	NULL	NULL	0	NULL	alcohol misuse	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The US Preventive Services Task Force recommends brief interventions for reducing alcohol misuse by adults , including pregnant women .
	manualset3
154843	4	408457	13	NULL	NULL	0	NULL	adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The US Preventive Services Task Force recommends brief interventions for reducing alcohol misuse by adults , including pregnant women .
	manualset3
154844	5	408457	13	NULL	NULL	0	NULL	pregnant women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The US Preventive Services Task Force recommends brief interventions for reducing alcohol misuse by adults , including pregnant women .
	manualset3
154845	1	408458	13	NULL	NULL	0	NULL	USB desmosome frequency	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The USB desmosome frequency in PKP1 null patients was similar to the LSB compartment ( but reduced by 43 % compared to USB controls ) .
	manualset3
154846	2	408458	13	NULL	NULL	0	NULL	PKP1 null patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The USB desmosome frequency in PKP1 null patients was similar to the LSB compartment ( but reduced by 43 % compared to USB controls ) .
	manualset3
154847	3	408458	13	NULL	NULL	0	NULL	LSB compartment 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The USB desmosome frequency in PKP1 null patients was similar to the LSB compartment ( but reduced by 43 % compared to USB controls ) .
	manualset3
154848	4	408458	13	NULL	NULL	0	NULL	43 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The USB desmosome frequency in PKP1 null patients was similar to the LSB compartment ( but reduced by 43 % compared to USB controls ) .
	manualset3
154849	5	408458	13	NULL	NULL	0	NULL	USB controls 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The USB desmosome frequency in PKP1 null patients was similar to the LSB compartment ( but reduced by 43 % compared to USB controls ) .
	manualset3
154850	1	408459	13	NULL	NULL	0	NULL	UV absorbance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The UV absorbance of these toxins measured at 200 nm showed good linearity in the range of 6.25-200 microg/mL with R = 0.992 for OA and 0.997 for DTX-1 .
	manualset3
154851	2	408459	13	NULL	NULL	0	NULL	toxins 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The UV absorbance of these toxins measured at 200 nm showed good linearity in the range of 6.25-200 microg/mL with R = 0.992 for OA and 0.997 for DTX-1 .
	manualset3
154852	3	408459	13	NULL	NULL	0	NULL	200 nm 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The UV absorbance of these toxins measured at 200 nm showed good linearity in the range of 6.25-200 microg/mL with R = 0.992 for OA and 0.997 for DTX-1 .
	manualset3
154853	4	408459	13	NULL	NULL	0	NULL	linearity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The UV absorbance of these toxins measured at 200 nm showed good linearity in the range of 6.25-200 microg/mL with R = 0.992 for OA and 0.997 for DTX-1 .
	manualset3
154854	5	408459	13	NULL	NULL	0	NULL	range of 6.25-200 microg/mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The UV absorbance of these toxins measured at 200 nm showed good linearity in the range of 6.25-200 microg/mL with R = 0.992 for OA and 0.997 for DTX-1 .
	manualset3
154855	6	408459	13	NULL	NULL	0	NULL	R = 0.992 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The UV absorbance of these toxins measured at 200 nm showed good linearity in the range of 6.25-200 microg/mL with R = 0.992 for OA and 0.997 for DTX-1 .
	manualset3
154856	7	408459	13	NULL	NULL	0	NULL	OA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The UV absorbance of these toxins measured at 200 nm showed good linearity in the range of 6.25-200 microg/mL with R = 0.992 for OA and 0.997 for DTX-1 .
	manualset3
154857	8	408459	13	NULL	NULL	0	NULL	0.997 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The UV absorbance of these toxins measured at 200 nm showed good linearity in the range of 6.25-200 microg/mL with R = 0.992 for OA and 0.997 for DTX-1 .
	manualset3
154858	9	408459	13	NULL	NULL	0	NULL	DTX-1	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The UV absorbance of these toxins measured at 200 nm showed good linearity in the range of 6.25-200 microg/mL with R = 0.992 for OA and 0.997 for DTX-1 .
	manualset3
154859	1	408460	13	NULL	NULL	0	NULL	United Nations	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The United Nations and World Health Organization have produced targeted prevention strategies to control the pandemic that focus on comprehensive prevention activities and universal access to care .
	manualset3
154860	2	408460	13	NULL	NULL	0	NULL	World Health Organization	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The United Nations and World Health Organization have produced targeted prevention strategies to control the pandemic that focus on comprehensive prevention activities and universal access to care .
	manualset3
154861	3	408460	13	NULL	NULL	0	NULL	prevention strategies 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The United Nations and World Health Organization have produced targeted prevention strategies to control the pandemic that focus on comprehensive prevention activities and universal access to care .
	manualset3
154862	4	408460	13	NULL	NULL	0	NULL	pandemic	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The United Nations and World Health Organization have produced targeted prevention strategies to control the pandemic that focus on comprehensive prevention activities and universal access to care .
	manualset3
154863	5	408460	13	NULL	NULL	0	NULL	focus	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The United Nations and World Health Organization have produced targeted prevention strategies to control the pandemic that focus on comprehensive prevention activities and universal access to care .
	manualset3
154864	6	408460	13	NULL	NULL	0	NULL	prevention activities	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The United Nations and World Health Organization have produced targeted prevention strategies to control the pandemic that focus on comprehensive prevention activities and universal access to care .
	manualset3
154865	7	408460	13	NULL	NULL	0	NULL	universal access	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The United Nations and World Health Organization have produced targeted prevention strategies to control the pandemic that focus on comprehensive prevention activities and universal access to care .
	manualset3
154868	1	408461	13	NULL	NULL	0	NULL	decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3 ) The decrease of IK was progressive , while the change of INa always began after IK proceeded to decrease rapidly .
	manualset3
154869	2	408461	13	NULL	NULL	0	NULL	IK	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3 ) The decrease of IK was progressive , while the change of INa always began after IK proceeded to decrease rapidly .
	manualset3
154870	3	408461	13	NULL	NULL	0	NULL	change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3 ) The decrease of IK was progressive , while the change of INa always began after IK proceeded to decrease rapidly .
	manualset3
154871	4	408461	13	NULL	NULL	0	NULL	INa	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3 ) The decrease of IK was progressive , while the change of INa always began after IK proceeded to decrease rapidly .
	manualset3
154872	5	408461	13	NULL	NULL	0	NULL	IK 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3 ) The decrease of IK was progressive , while the change of INa always began after IK proceeded to decrease rapidly .
	manualset3
154873	1	408462	13	NULL	NULL	0	NULL	Characteristics 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Characteristics of the spread of bartonellosis and the measures for its prevention ) .
	manualset3
154874	2	408462	13	NULL	NULL	0	NULL	bartonellosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Characteristics of the spread of bartonellosis and the measures for its prevention ) .
	manualset3
154875	3	408462	13	NULL	NULL	0	NULL	prevention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Characteristics of the spread of bartonellosis and the measures for its prevention ) .
	manualset3
157259	4	408462	13	NULL	NULL	0	NULL	measures 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Characteristics of the spread of bartonellosis and the measures for its prevention ) .
	manualset3
154876	1	408463	13	NULL	NULL	0	NULL	safe way 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A reliable and safe way of shortening cadaver kidney ischemia time : prenephrectomy tissue typing using donor lymph node cells .
	manualset3
154877	2	408463	13	NULL	NULL	0	NULL	cadaver kidney ischemia time	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A reliable and safe way of shortening cadaver kidney ischemia time : prenephrectomy tissue typing using donor lymph node cells .
	manualset3
154878	3	408463	13	NULL	NULL	0	NULL	prenephrectomy tissue typing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A reliable and safe way of shortening cadaver kidney ischemia time : prenephrectomy tissue typing using donor lymph node cells .
	manualset3
154879	4	408463	13	NULL	NULL	0	NULL	donor lymph node cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A reliable and safe way of shortening cadaver kidney ischemia time : prenephrectomy tissue typing using donor lymph node cells .
	manualset3
154880	1	408464	13	NULL	NULL	0	NULL	Use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Use of Wolfe Grafts and Tendon-Lengthening in Treating Cicatricial Contractures .
	manualset3
154881	2	408464	13	NULL	NULL	0	NULL	Wolfe Grafts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The Use of Wolfe Grafts and Tendon-Lengthening in Treating Cicatricial Contractures .
	manualset3
154882	3	408464	13	NULL	NULL	0	NULL	Cicatricial Contractures 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Use of Wolfe Grafts and Tendon-Lengthening in Treating Cicatricial Contractures .
	manualset3
154883	1	408465	13	NULL	NULL	0	NULL	 VCAM-1 expressing cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The VCAM-1 expressing cells were mainly present in the synovial lining layer .
	manualset3
154884	2	408465	13	NULL	NULL	0	NULL	synovial lining layer	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The VCAM-1 expressing cells were mainly present in the synovial lining layer .
	manualset3
154885	1	408466	13	NULL	NULL	0	NULL	VITEK ( ) 2 system	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The VITEK ( ) 2 system and E-tests were used to determine the minimum inhibitory concentrations needed to inhibit bacterial growth .
	manualset3
154886	2	408466	13	NULL	NULL	0	NULL	E-tests	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The VITEK ( ) 2 system and E-tests were used to determine the minimum inhibitory concentrations needed to inhibit bacterial growth .
	manualset3
154887	3	408466	13	NULL	NULL	0	NULL	minimum inhibitory concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The VITEK ( ) 2 system and E-tests were used to determine the minimum inhibitory concentrations needed to inhibit bacterial growth .
	manualset3
154888	4	408466	13	NULL	NULL	0	NULL	bacterial growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The VITEK ( ) 2 system and E-tests were used to determine the minimum inhibitory concentrations needed to inhibit bacterial growth .
	manualset3
154889	1	408467	13	NULL	NULL	0	NULL	VOCs	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The VOCs were reconstructed from a varying number of images ( 10-66 images ) and compared to the CBCT ground truth using four different metrics ( mean squared error , correlation coefficient , structural similarity index and perceptual difference model ) .
	manualset3
154890	2	408467	13	NULL	NULL	0	NULL	number of images	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The VOCs were reconstructed from a varying number of images ( 10-66 images ) and compared to the CBCT ground truth using four different metrics ( mean squared error , correlation coefficient , structural similarity index and perceptual difference model ) .
	manualset3
154891	3	408467	13	NULL	NULL	0	NULL	10-66 images	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The VOCs were reconstructed from a varying number of images ( 10-66 images ) and compared to the CBCT ground truth using four different metrics ( mean squared error , correlation coefficient , structural similarity index and perceptual difference model ) .
	manualset3
154892	4	408467	13	NULL	NULL	0	NULL	 CBCT	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The VOCs were reconstructed from a varying number of images ( 10-66 images ) and compared to the CBCT ground truth using four different metrics ( mean squared error , correlation coefficient , structural similarity index and perceptual difference model ) .
	manualset3
154893	5	408467	13	NULL	NULL	0	NULL	ground truth	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The VOCs were reconstructed from a varying number of images ( 10-66 images ) and compared to the CBCT ground truth using four different metrics ( mean squared error , correlation coefficient , structural similarity index and perceptual difference model ) .
	manualset3
154894	6	408467	13	NULL	NULL	0	NULL	metrics	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The VOCs were reconstructed from a varying number of images ( 10-66 images ) and compared to the CBCT ground truth using four different metrics ( mean squared error , correlation coefficient , structural similarity index and perceptual difference model ) .
	manualset3
154895	7	408467	13	NULL	NULL	0	NULL	mean squared error	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The VOCs were reconstructed from a varying number of images ( 10-66 images ) and compared to the CBCT ground truth using four different metrics ( mean squared error , correlation coefficient , structural similarity index and perceptual difference model ) .
	manualset3
154896	8	408467	13	NULL	NULL	0	NULL	 correlation coefficient 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The VOCs were reconstructed from a varying number of images ( 10-66 images ) and compared to the CBCT ground truth using four different metrics ( mean squared error , correlation coefficient , structural similarity index and perceptual difference model ) .
	manualset3
154897	9	408467	13	NULL	NULL	0	NULL	structural similarity index 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The VOCs were reconstructed from a varying number of images ( 10-66 images ) and compared to the CBCT ground truth using four different metrics ( mean squared error , correlation coefficient , structural similarity index and perceptual difference model ) .
	manualset3
154898	10	408467	13	NULL	NULL	0	NULL	perceptual difference model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The VOCs were reconstructed from a varying number of images ( 10-66 images ) and compared to the CBCT ground truth using four different metrics ( mean squared error , correlation coefficient , structural similarity index and perceptual difference model ) .
	manualset3
154899	1	408468	13	NULL	NULL	0	NULL	VPg 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The VPg ( approximately 25 kDa ) only , and not the unprocessed NIa , was detected .
	manualset3
154900	2	408468	13	NULL	NULL	0	NULL	approximately 25 kDa	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The VPg ( approximately 25 kDa ) only , and not the unprocessed NIa , was detected .
	manualset3
154901	3	408468	13	NULL	NULL	0	NULL	unprocessed NIa	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The VPg ( approximately 25 kDa ) only , and not the unprocessed NIa , was detected .
	manualset3
154902	1	408469	13	NULL	NULL	0	NULL	VWF bead-induced platelet activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The VWF bead-induced platelet activation was completely inhibited by addition of monoclonal antibody ( mAb ) to GPIb or GPIIb/IIIa .
	manualset3
154903	2	408469	13	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The VWF bead-induced platelet activation was completely inhibited by addition of monoclonal antibody ( mAb ) to GPIb or GPIIb/IIIa .
	manualset3
154904	3	408469	13	NULL	NULL	0	NULL	monoclonal antibody ( mAb )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The VWF bead-induced platelet activation was completely inhibited by addition of monoclonal antibody ( mAb ) to GPIb or GPIIb/IIIa .
	manualset3
154905	4	408469	13	NULL	NULL	0	NULL	GPIb	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The VWF bead-induced platelet activation was completely inhibited by addition of monoclonal antibody ( mAb ) to GPIb or GPIIb/IIIa .
	manualset3
154906	5	408469	13	NULL	NULL	0	NULL	GPIIb/IIIa	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The VWF bead-induced platelet activation was completely inhibited by addition of monoclonal antibody ( mAb ) to GPIb or GPIIb/IIIa .
	manualset3
154907	1	408470	13	NULL	NULL	0	NULL	Vmax	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Vmax for the phosphorothioate analog was approximately half that for the phosphate derivative .
	manualset3
154908	2	408470	13	NULL	NULL	0	NULL	phosphorothioate analog	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The Vmax for the phosphorothioate analog was approximately half that for the phosphate derivative .
	manualset3
154909	3	408470	13	NULL	NULL	0	NULL	approximately half	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Vmax for the phosphorothioate analog was approximately half that for the phosphate derivative .
	manualset3
154910	4	408470	13	NULL	NULL	0	NULL	phosphate derivative	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The Vmax for the phosphorothioate analog was approximately half that for the phosphate derivative .
	manualset3
154911	1	408471	13	NULL	NULL	0	NULL	 World Health Organization ( WHO )	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The World Health Organization ( WHO ) classification of tumors of hematopoietic and lymphoid tissues ( 2001 ) defined a provisional entity named refractory anemia with ringed sideroblasts associated to marked thrombocytosis ( RARS-MT ) .
	manualset3
154912	2	408471	13	NULL	NULL	0	NULL	classification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The World Health Organization ( WHO ) classification of tumors of hematopoietic and lymphoid tissues ( 2001 ) defined a provisional entity named refractory anemia with ringed sideroblasts associated to marked thrombocytosis ( RARS-MT ) .
	manualset3
154913	3	408471	13	NULL	NULL	0	NULL	tumors of hematopoietic tissues 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The World Health Organization ( WHO ) classification of tumors of hematopoietic and lymphoid tissues ( 2001 ) defined a provisional entity named refractory anemia with ringed sideroblasts associated to marked thrombocytosis ( RARS-MT ) .
	manualset3
154914	4	408471	13	NULL	NULL	0	NULL	tumors of lymphoid tissues 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The World Health Organization ( WHO ) classification of tumors of hematopoietic and lymphoid tissues ( 2001 ) defined a provisional entity named refractory anemia with ringed sideroblasts associated to marked thrombocytosis ( RARS-MT ) .
	manualset3
154915	5	408471	13	NULL	NULL	0	NULL	2001	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The World Health Organization ( WHO ) classification of tumors of hematopoietic and lymphoid tissues ( 2001 ) defined a provisional entity named refractory anemia with ringed sideroblasts associated to marked thrombocytosis ( RARS-MT ) .
	manualset3
154916	6	408471	13	NULL	NULL	0	NULL	 provisional entity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The World Health Organization ( WHO ) classification of tumors of hematopoietic and lymphoid tissues ( 2001 ) defined a provisional entity named refractory anemia with ringed sideroblasts associated to marked thrombocytosis ( RARS-MT ) .
	manualset3
154917	7	408471	13	NULL	NULL	0	NULL	refractory anemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The World Health Organization ( WHO ) classification of tumors of hematopoietic and lymphoid tissues ( 2001 ) defined a provisional entity named refractory anemia with ringed sideroblasts associated to marked thrombocytosis ( RARS-MT ) .
	manualset3
154918	8	408471	13	NULL	NULL	0	NULL	ringed sideroblasts associated to marked thrombocytosis ( RARS-MT ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The World Health Organization ( WHO ) classification of tumors of hematopoietic and lymphoid tissues ( 2001 ) defined a provisional entity named refractory anemia with ringed sideroblasts associated to marked thrombocytosis ( RARS-MT ) .
	manualset3
154919	1	408472	13	NULL	NULL	0	NULL	X-ray Photoelectron Spectroscopy ( XPS ) analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The X-ray Photoelectron Spectroscopy ( XPS ) analysis , together with gas chromatography-mass spectrometry ( GC-MS ) and Fourier Transform Infrared spectroscopy ( FT-IR ) analysis , prove that nearly all the initial fluorine residing in the gas phase is in the form of SiF4 , whereas , the initial sulfur is deposited in the form of elemental sulfur , after photodegradation .
	manualset3
154920	2	408472	13	NULL	NULL	0	NULL	gas chromatography-mass spectrometry ( GC-MS )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The X-ray Photoelectron Spectroscopy ( XPS ) analysis , together with gas chromatography-mass spectrometry ( GC-MS ) and Fourier Transform Infrared spectroscopy ( FT-IR ) analysis , prove that nearly all the initial fluorine residing in the gas phase is in the form of SiF4 , whereas , the initial sulfur is deposited in the form of elemental sulfur , after photodegradation .
	manualset3
154921	3	408472	13	NULL	NULL	0	NULL	Fourier Transform Infrared spectroscopy ( FT-IR ) analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The X-ray Photoelectron Spectroscopy ( XPS ) analysis , together with gas chromatography-mass spectrometry ( GC-MS ) and Fourier Transform Infrared spectroscopy ( FT-IR ) analysis , prove that nearly all the initial fluorine residing in the gas phase is in the form of SiF4 , whereas , the initial sulfur is deposited in the form of elemental sulfur , after photodegradation .
	manualset3
154922	4	408472	13	NULL	NULL	0	NULL	fluorine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The X-ray Photoelectron Spectroscopy ( XPS ) analysis , together with gas chromatography-mass spectrometry ( GC-MS ) and Fourier Transform Infrared spectroscopy ( FT-IR ) analysis , prove that nearly all the initial fluorine residing in the gas phase is in the form of SiF4 , whereas , the initial sulfur is deposited in the form of elemental sulfur , after photodegradation .
	manualset3
154923	5	408472	13	NULL	NULL	0	NULL	gas phase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The X-ray Photoelectron Spectroscopy ( XPS ) analysis , together with gas chromatography-mass spectrometry ( GC-MS ) and Fourier Transform Infrared spectroscopy ( FT-IR ) analysis , prove that nearly all the initial fluorine residing in the gas phase is in the form of SiF4 , whereas , the initial sulfur is deposited in the form of elemental sulfur , after photodegradation .
	manualset3
154924	6	408472	13	NULL	NULL	0	NULL	form 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The X-ray Photoelectron Spectroscopy ( XPS ) analysis , together with gas chromatography-mass spectrometry ( GC-MS ) and Fourier Transform Infrared spectroscopy ( FT-IR ) analysis , prove that nearly all the initial fluorine residing in the gas phase is in the form of SiF4 , whereas , the initial sulfur is deposited in the form of elemental sulfur , after photodegradation .
	manualset3
154925	7	408472	13	NULL	NULL	0	NULL	SiF4	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The X-ray Photoelectron Spectroscopy ( XPS ) analysis , together with gas chromatography-mass spectrometry ( GC-MS ) and Fourier Transform Infrared spectroscopy ( FT-IR ) analysis , prove that nearly all the initial fluorine residing in the gas phase is in the form of SiF4 , whereas , the initial sulfur is deposited in the form of elemental sulfur , after photodegradation .
	manualset3
154926	8	408472	13	NULL	NULL	0	NULL	sulfur	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The X-ray Photoelectron Spectroscopy ( XPS ) analysis , together with gas chromatography-mass spectrometry ( GC-MS ) and Fourier Transform Infrared spectroscopy ( FT-IR ) analysis , prove that nearly all the initial fluorine residing in the gas phase is in the form of SiF4 , whereas , the initial sulfur is deposited in the form of elemental sulfur , after photodegradation .
	manualset3
154927	9	408472	13	NULL	NULL	0	NULL	form 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The X-ray Photoelectron Spectroscopy ( XPS ) analysis , together with gas chromatography-mass spectrometry ( GC-MS ) and Fourier Transform Infrared spectroscopy ( FT-IR ) analysis , prove that nearly all the initial fluorine residing in the gas phase is in the form of SiF4 , whereas , the initial sulfur is deposited in the form of elemental sulfur , after photodegradation .
	manualset3
154928	10	408472	13	NULL	NULL	NULL	NULL	sulfur	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The X-ray Photoelectron Spectroscopy ( XPS ) analysis , together with gas chromatography-mass spectrometry ( GC-MS ) and Fourier Transform Infrared spectroscopy ( FT-IR ) analysis , prove that nearly all the initial fluorine residing in the gas phase is in the form of SiF4 , whereas , the initial sulfur is deposited in the form of elemental sulfur , after photodegradation .
	manualset3
154929	11	408472	13	NULL	NULL	0	NULL	photodegradation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The X-ray Photoelectron Spectroscopy ( XPS ) analysis , together with gas chromatography-mass spectrometry ( GC-MS ) and Fourier Transform Infrared spectroscopy ( FT-IR ) analysis , prove that nearly all the initial fluorine residing in the gas phase is in the form of SiF4 , whereas , the initial sulfur is deposited in the form of elemental sulfur , after photodegradation .
	manualset3
154930	1	408473	13	NULL	NULL	0	NULL	 Zoladex Early Breast Cancer Research Association ( ZEBRA ) trial	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Zoladex Early Breast Cancer Research Association ( ZEBRA ) trial compared the efficacy and tolerability of goserelin ( Zoladex ) with cyclophosphamide , methotrexate and 5-fluorouracil ( CMF ) chemotherapy in pre - / perimenopausal women with node-positive early breast cancer .
	manualset3
154931	2	408473	13	NULL	NULL	0	NULL	efficacy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Zoladex Early Breast Cancer Research Association ( ZEBRA ) trial compared the efficacy and tolerability of goserelin ( Zoladex ) with cyclophosphamide , methotrexate and 5-fluorouracil ( CMF ) chemotherapy in pre - / perimenopausal women with node-positive early breast cancer .
	manualset3
154932	3	408473	13	NULL	NULL	0	NULL	tolerability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Zoladex Early Breast Cancer Research Association ( ZEBRA ) trial compared the efficacy and tolerability of goserelin ( Zoladex ) with cyclophosphamide , methotrexate and 5-fluorouracil ( CMF ) chemotherapy in pre - / perimenopausal women with node-positive early breast cancer .
	manualset3
154933	4	408473	13	NULL	NULL	0	NULL	 goserelin ( Zoladex ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The Zoladex Early Breast Cancer Research Association ( ZEBRA ) trial compared the efficacy and tolerability of goserelin ( Zoladex ) with cyclophosphamide , methotrexate and 5-fluorouracil ( CMF ) chemotherapy in pre - / perimenopausal women with node-positive early breast cancer .
	manualset3
154934	5	408473	13	NULL	NULL	0	NULL	cyclophosphamide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The Zoladex Early Breast Cancer Research Association ( ZEBRA ) trial compared the efficacy and tolerability of goserelin ( Zoladex ) with cyclophosphamide , methotrexate and 5-fluorouracil ( CMF ) chemotherapy in pre - / perimenopausal women with node-positive early breast cancer .
	manualset3
154935	6	408473	13	NULL	NULL	0	NULL	methotrexate	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The Zoladex Early Breast Cancer Research Association ( ZEBRA ) trial compared the efficacy and tolerability of goserelin ( Zoladex ) with cyclophosphamide , methotrexate and 5-fluorouracil ( CMF ) chemotherapy in pre - / perimenopausal women with node-positive early breast cancer .
	manualset3
154936	7	408473	13	NULL	NULL	0	NULL	5-fluorouracil 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The Zoladex Early Breast Cancer Research Association ( ZEBRA ) trial compared the efficacy and tolerability of goserelin ( Zoladex ) with cyclophosphamide , methotrexate and 5-fluorouracil ( CMF ) chemotherapy in pre - / perimenopausal women with node-positive early breast cancer .
	manualset3
154937	8	408473	13	NULL	NULL	0	NULL	CMF	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The Zoladex Early Breast Cancer Research Association ( ZEBRA ) trial compared the efficacy and tolerability of goserelin ( Zoladex ) with cyclophosphamide , methotrexate and 5-fluorouracil ( CMF ) chemotherapy in pre - / perimenopausal women with node-positive early breast cancer .
	manualset3
154938	9	408473	13	NULL	NULL	0	NULL	chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The Zoladex Early Breast Cancer Research Association ( ZEBRA ) trial compared the efficacy and tolerability of goserelin ( Zoladex ) with cyclophosphamide , methotrexate and 5-fluorouracil ( CMF ) chemotherapy in pre - / perimenopausal women with node-positive early breast cancer .
	manualset3
154939	10	408473	13	NULL	NULL	0	NULL	pre - / perimenopausal women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The Zoladex Early Breast Cancer Research Association ( ZEBRA ) trial compared the efficacy and tolerability of goserelin ( Zoladex ) with cyclophosphamide , methotrexate and 5-fluorouracil ( CMF ) chemotherapy in pre - / perimenopausal women with node-positive early breast cancer .
	manualset3
154940	11	408473	13	NULL	NULL	0	NULL	 breast cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The Zoladex Early Breast Cancer Research Association ( ZEBRA ) trial compared the efficacy and tolerability of goserelin ( Zoladex ) with cyclophosphamide , methotrexate and 5-fluorouracil ( CMF ) chemotherapy in pre - / perimenopausal women with node-positive early breast cancer .
	manualset3
154941	1	408474	13	NULL	NULL	0	NULL	` Organic ' product label	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The ` Organic ' product label guarantees a production process that avoids the use of synthetic fertilisers , pesticides and hormones and minimises recourse to pharmaceuticals or veterinary drugs ; however , the product 's quality remains an issue that needs to be addressed in response to consumer demand .
	manualset3
154942	2	408474	13	NULL	NULL	0	NULL	production process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ` Organic ' product label guarantees a production process that avoids the use of synthetic fertilisers , pesticides and hormones and minimises recourse to pharmaceuticals or veterinary drugs ; however , the product 's quality remains an issue that needs to be addressed in response to consumer demand .
	manualset3
154943	3	408474	13	NULL	NULL	0	NULL	use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ` Organic ' product label guarantees a production process that avoids the use of synthetic fertilisers , pesticides and hormones and minimises recourse to pharmaceuticals or veterinary drugs ; however , the product 's quality remains an issue that needs to be addressed in response to consumer demand .
	manualset3
154944	4	408474	13	NULL	NULL	0	NULL	synthetic fertilisers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ` Organic ' product label guarantees a production process that avoids the use of synthetic fertilisers , pesticides and hormones and minimises recourse to pharmaceuticals or veterinary drugs ; however , the product 's quality remains an issue that needs to be addressed in response to consumer demand .
	manualset3
154945	5	408474	13	NULL	NULL	0	NULL	pesticides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ` Organic ' product label guarantees a production process that avoids the use of synthetic fertilisers , pesticides and hormones and minimises recourse to pharmaceuticals or veterinary drugs ; however , the product 's quality remains an issue that needs to be addressed in response to consumer demand .
	manualset3
154946	6	408474	13	NULL	NULL	0	NULL	hormones	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ` Organic ' product label guarantees a production process that avoids the use of synthetic fertilisers , pesticides and hormones and minimises recourse to pharmaceuticals or veterinary drugs ; however , the product 's quality remains an issue that needs to be addressed in response to consumer demand .
	manualset3
154947	7	408474	13	NULL	NULL	0	NULL	minimises 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ` Organic ' product label guarantees a production process that avoids the use of synthetic fertilisers , pesticides and hormones and minimises recourse to pharmaceuticals or veterinary drugs ; however , the product 's quality remains an issue that needs to be addressed in response to consumer demand .
	manualset3
154948	8	408474	13	NULL	NULL	0	NULL	recourse	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ` Organic ' product label guarantees a production process that avoids the use of synthetic fertilisers , pesticides and hormones and minimises recourse to pharmaceuticals or veterinary drugs ; however , the product 's quality remains an issue that needs to be addressed in response to consumer demand .
	manualset3
154949	9	408474	13	NULL	NULL	0	NULL	pharmaceuticals	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The ` Organic ' product label guarantees a production process that avoids the use of synthetic fertilisers , pesticides and hormones and minimises recourse to pharmaceuticals or veterinary drugs ; however , the product 's quality remains an issue that needs to be addressed in response to consumer demand .
	manualset3
154950	10	408474	13	NULL	NULL	0	NULL	 veterinary drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The ` Organic ' product label guarantees a production process that avoids the use of synthetic fertilisers , pesticides and hormones and minimises recourse to pharmaceuticals or veterinary drugs ; however , the product 's quality remains an issue that needs to be addressed in response to consumer demand .
	manualset3
154951	11	408474	13	NULL	NULL	0	NULL	product 's quality	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ` Organic ' product label guarantees a production process that avoids the use of synthetic fertilisers , pesticides and hormones and minimises recourse to pharmaceuticals or veterinary drugs ; however , the product 's quality remains an issue that needs to be addressed in response to consumer demand .
	manualset3
154952	12	408474	13	NULL	NULL	0	NULL	issue	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ` Organic ' product label guarantees a production process that avoids the use of synthetic fertilisers , pesticides and hormones and minimises recourse to pharmaceuticals or veterinary drugs ; however , the product 's quality remains an issue that needs to be addressed in response to consumer demand .
	manualset3
154953	13	408474	13	NULL	NULL	0	NULL	 response	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ` Organic ' product label guarantees a production process that avoids the use of synthetic fertilisers , pesticides and hormones and minimises recourse to pharmaceuticals or veterinary drugs ; however , the product 's quality remains an issue that needs to be addressed in response to consumer demand .
	manualset3
154954	14	408474	13	NULL	NULL	0	NULL	consumer demand	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ` Organic ' product label guarantees a production process that avoids the use of synthetic fertilisers , pesticides and hormones and minimises recourse to pharmaceuticals or veterinary drugs ; however , the product 's quality remains an issue that needs to be addressed in response to consumer demand .
	manualset3
154955	1	408475	13	NULL	NULL	0	NULL	 ` buckling ' theory	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The ` buckling ' theory contends that the fracture is produced as a result of transmission of force to the orbital floor from a blow to the orbital rim ( Fig .
	manualset3
154956	2	408475	13	NULL	NULL	0	NULL	fracture	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The ` buckling ' theory contends that the fracture is produced as a result of transmission of force to the orbital floor from a blow to the orbital rim ( Fig .
	manualset3
154957	3	408475	13	NULL	NULL	0	NULL	result	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The ` buckling ' theory contends that the fracture is produced as a result of transmission of force to the orbital floor from a blow to the orbital rim ( Fig .
	manualset3
154958	4	408475	13	NULL	NULL	0	NULL	transmission of force	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ` buckling ' theory contends that the fracture is produced as a result of transmission of force to the orbital floor from a blow to the orbital rim ( Fig .
	manualset3
154959	5	408475	13	NULL	NULL	0	NULL	orbital floor	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The ` buckling ' theory contends that the fracture is produced as a result of transmission of force to the orbital floor from a blow to the orbital rim ( Fig .
	manualset3
154960	6	408475	13	NULL	NULL	0	NULL	 blow	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ` buckling ' theory contends that the fracture is produced as a result of transmission of force to the orbital floor from a blow to the orbital rim ( Fig .
	manualset3
154961	7	408475	13	NULL	NULL	0	NULL	orbital rim	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The ` buckling ' theory contends that the fracture is produced as a result of transmission of force to the orbital floor from a blow to the orbital rim ( Fig .
	manualset3
155018	1	408476	13	NULL	NULL	0	NULL	European Guidelines	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The `` European Guidelines on Quality Criteria for Diagnostic Radiographic Images '' do not address the choice of the film characteristic ( H & D ) curve , which is an important parameter for the description of a radiographic screen-film system .
	manualset3
155019	2	408476	13	NULL	NULL	0	NULL	Quality Criteria	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The `` European Guidelines on Quality Criteria for Diagnostic Radiographic Images '' do not address the choice of the film characteristic ( H & D ) curve , which is an important parameter for the description of a radiographic screen-film system .
	manualset3
155020	3	408476	13	NULL	NULL	0	NULL	Diagnostic Radiographic Images	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The `` European Guidelines on Quality Criteria for Diagnostic Radiographic Images '' do not address the choice of the film characteristic ( H & D ) curve , which is an important parameter for the description of a radiographic screen-film system .
	manualset3
155021	4	408476	13	NULL	NULL	0	NULL	choice 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The `` European Guidelines on Quality Criteria for Diagnostic Radiographic Images '' do not address the choice of the film characteristic ( H & D ) curve , which is an important parameter for the description of a radiographic screen-film system .
	manualset3
155022	5	408476	13	NULL	NULL	0	NULL	film characteristic ( H & D ) curve	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The `` European Guidelines on Quality Criteria for Diagnostic Radiographic Images '' do not address the choice of the film characteristic ( H & D ) curve , which is an important parameter for the description of a radiographic screen-film system .
	manualset3
155023	6	408476	13	NULL	NULL	0	NULL	parameter	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The `` European Guidelines on Quality Criteria for Diagnostic Radiographic Images '' do not address the choice of the film characteristic ( H & D ) curve , which is an important parameter for the description of a radiographic screen-film system .
	manualset3
155024	7	408476	13	NULL	NULL	0	NULL	description	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The `` European Guidelines on Quality Criteria for Diagnostic Radiographic Images '' do not address the choice of the film characteristic ( H & D ) curve , which is an important parameter for the description of a radiographic screen-film system .
	manualset3
155025	8	408476	13	NULL	NULL	0	NULL	radiographic screen-film system	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The `` European Guidelines on Quality Criteria for Diagnostic Radiographic Images '' do not address the choice of the film characteristic ( H & D ) curve , which is an important parameter for the description of a radiographic screen-film system .
	manualset3
155026	1	408477	13	NULL	NULL	0	NULL	T - cell nature	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The `` T - '' or `` B - '' cell nature of the ocular FcR and their possible functions in regulating ocular immune responses are yet to be determined .
	manualset3
155027	2	408477	13	NULL	NULL	0	NULL	`` B - '' cell nature	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The `` T - '' or `` B - '' cell nature of the ocular FcR and their possible functions in regulating ocular immune responses are yet to be determined .
	manualset3
155028	3	408477	13	NULL	NULL	0	NULL	ocular FcR 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The `` T - '' or `` B - '' cell nature of the ocular FcR and their possible functions in regulating ocular immune responses are yet to be determined .
	manualset3
155029	4	408477	13	NULL	NULL	0	NULL	functions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The `` T - '' or `` B - '' cell nature of the ocular FcR and their possible functions in regulating ocular immune responses are yet to be determined .
	manualset3
155030	5	408477	13	NULL	NULL	0	NULL	ocular immune responses 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The `` T - '' or `` B - '' cell nature of the ocular FcR and their possible functions in regulating ocular immune responses are yet to be determined .
	manualset3
155031	1	408478	13	NULL	NULL	0	NULL	`` alpha '' form of HC 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The `` alpha '' form of HC is the standard 2C form with a MW of 40 Kd .
	manualset3
155032	2	408478	13	NULL	NULL	0	NULL	2C form	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The `` alpha '' form of HC is the standard 2C form with a MW of 40 Kd .
	manualset3
155033	3	408478	13	NULL	NULL	0	NULL	MW of 40 Kd 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The `` alpha '' form of HC is the standard 2C form with a MW of 40 Kd .
	manualset3
155034	1	408479	13	NULL	NULL	0	NULL	abdominal sonogram	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The abdominal sonogram showed an unusual position of the spleen in the left-lower quadrant , with no splenic ischemia .
	manualset3
155035	2	408479	13	NULL	NULL	0	NULL	unusual position	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The abdominal sonogram showed an unusual position of the spleen in the left-lower quadrant , with no splenic ischemia .
	manualset3
155036	3	408479	13	NULL	NULL	0	NULL	spleen 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The abdominal sonogram showed an unusual position of the spleen in the left-lower quadrant , with no splenic ischemia .
	manualset3
155037	4	408479	13	NULL	NULL	0	NULL	left-lower quadrant	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The abdominal sonogram showed an unusual position of the spleen in the left-lower quadrant , with no splenic ischemia .
	manualset3
155038	5	408479	13	NULL	NULL	0	NULL	splenic ischemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The abdominal sonogram showed an unusual position of the spleen in the left-lower quadrant , with no splenic ischemia .
	manualset3
155039	1	408480	13	NULL	NULL	0	NULL	transcript 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The aberrant transcript is predicted to encode a truncated p53 protein containing 189 amino acid residues .
	manualset3
155040	2	408480	13	NULL	NULL	0	NULL	 p53 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The aberrant transcript is predicted to encode a truncated p53 protein containing 189 amino acid residues .
	manualset3
155041	3	408480	13	NULL	NULL	0	NULL	189 amino acid residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The aberrant transcript is predicted to encode a truncated p53 protein containing 189 amino acid residues .
	manualset3
155042	1	408481	13	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of APC to shuttle between these and other cell locations is hypothesized to be integral to its cellular function .
	manualset3
155043	2	408481	13	NULL	NULL	0	NULL	APC	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of APC to shuttle between these and other cell locations is hypothesized to be integral to its cellular function .
	manualset3
155044	3	408481	13	NULL	NULL	0	NULL	cell locations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of APC to shuttle between these and other cell locations is hypothesized to be integral to its cellular function .
	manualset3
155045	4	408481	13	NULL	NULL	0	NULL	cellular function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of APC to shuttle between these and other cell locations is hypothesized to be integral to its cellular function .
	manualset3
155046	1	408482	13	NULL	NULL	0	NULL	ability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of Dupuytren 's fibroblasts to generate contractile force was determined by using a previously described collagen lattice contraction assay .
	manualset3
155047	2	408482	13	NULL	NULL	0	NULL	Dupuytren 's fibroblasts	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of Dupuytren 's fibroblasts to generate contractile force was determined by using a previously described collagen lattice contraction assay .
	manualset3
155048	3	408482	13	NULL	NULL	0	NULL	contractile force	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of Dupuytren 's fibroblasts to generate contractile force was determined by using a previously described collagen lattice contraction assay .
	manualset3
155049	4	408482	13	NULL	NULL	0	NULL	collagen lattice contraction assay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of Dupuytren 's fibroblasts to generate contractile force was determined by using a previously described collagen lattice contraction assay .
	manualset3
155050	1	408483	13	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of EtxB to alter immune reactivity is dependent on its ability to modulate immune cell function through binding to cell surface molecules , the principal receptor of which is the ubiquitous GM1-ganglioside .
	manualset3
155051	2	408483	13	NULL	NULL	0	NULL	EtxB	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of EtxB to alter immune reactivity is dependent on its ability to modulate immune cell function through binding to cell surface molecules , the principal receptor of which is the ubiquitous GM1-ganglioside .
	manualset3
155052	3	408483	13	NULL	NULL	0	NULL	immune reactivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of EtxB to alter immune reactivity is dependent on its ability to modulate immune cell function through binding to cell surface molecules , the principal receptor of which is the ubiquitous GM1-ganglioside .
	manualset3
155053	4	408483	13	NULL	NULL	0	NULL	immune cell function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of EtxB to alter immune reactivity is dependent on its ability to modulate immune cell function through binding to cell surface molecules , the principal receptor of which is the ubiquitous GM1-ganglioside .
	manualset3
155054	5	408483	13	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of EtxB to alter immune reactivity is dependent on its ability to modulate immune cell function through binding to cell surface molecules , the principal receptor of which is the ubiquitous GM1-ganglioside .
	manualset3
155055	6	408483	13	NULL	NULL	0	NULL	cell surface molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of EtxB to alter immune reactivity is dependent on its ability to modulate immune cell function through binding to cell surface molecules , the principal receptor of which is the ubiquitous GM1-ganglioside .
	manualset3
155056	7	408483	13	NULL	NULL	0	NULL	receptor	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of EtxB to alter immune reactivity is dependent on its ability to modulate immune cell function through binding to cell surface molecules , the principal receptor of which is the ubiquitous GM1-ganglioside .
	manualset3
155057	8	408483	13	NULL	NULL	0	NULL	ubiquitous GM1-ganglioside	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of EtxB to alter immune reactivity is dependent on its ability to modulate immune cell function through binding to cell surface molecules , the principal receptor of which is the ubiquitous GM1-ganglioside .
	manualset3
155058	1	408484	13	NULL	NULL	0	NULL	ability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of MnTMPyP to restore nitrergic neurotransmission may therefore provide a lead in the development of SOD mimetics as therapeutic agents in the treatment of neuropathies associated with oxidant stress .
	manualset3
155059	2	408484	13	NULL	NULL	0	NULL	MnTMPyP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of MnTMPyP to restore nitrergic neurotransmission may therefore provide a lead in the development of SOD mimetics as therapeutic agents in the treatment of neuropathies associated with oxidant stress .
	manualset3
155060	3	408484	13	NULL	NULL	0	NULL	nitrergic neurotransmission	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of MnTMPyP to restore nitrergic neurotransmission may therefore provide a lead in the development of SOD mimetics as therapeutic agents in the treatment of neuropathies associated with oxidant stress .
	manualset3
155061	4	408484	13	NULL	NULL	0	NULL	lead	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of MnTMPyP to restore nitrergic neurotransmission may therefore provide a lead in the development of SOD mimetics as therapeutic agents in the treatment of neuropathies associated with oxidant stress .
	manualset3
155062	5	408484	13	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of MnTMPyP to restore nitrergic neurotransmission may therefore provide a lead in the development of SOD mimetics as therapeutic agents in the treatment of neuropathies associated with oxidant stress .
	manualset3
155063	6	408484	13	NULL	NULL	0	NULL	SOD mimetics	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of MnTMPyP to restore nitrergic neurotransmission may therefore provide a lead in the development of SOD mimetics as therapeutic agents in the treatment of neuropathies associated with oxidant stress .
	manualset3
155064	7	408484	13	NULL	NULL	0	NULL	therapeutic agents 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of MnTMPyP to restore nitrergic neurotransmission may therefore provide a lead in the development of SOD mimetics as therapeutic agents in the treatment of neuropathies associated with oxidant stress .
	manualset3
155065	8	408484	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of MnTMPyP to restore nitrergic neurotransmission may therefore provide a lead in the development of SOD mimetics as therapeutic agents in the treatment of neuropathies associated with oxidant stress .
	manualset3
155066	9	408484	13	NULL	NULL	0	NULL	neuropathies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of MnTMPyP to restore nitrergic neurotransmission may therefore provide a lead in the development of SOD mimetics as therapeutic agents in the treatment of neuropathies associated with oxidant stress .
	manualset3
155067	10	408484	13	NULL	NULL	0	NULL	oxidant stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of MnTMPyP to restore nitrergic neurotransmission may therefore provide a lead in the development of SOD mimetics as therapeutic agents in the treatment of neuropathies associated with oxidant stress .
	manualset3
155068	1	408485	13	NULL	NULL	0	NULL	ability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of Paraconiothyrium variabile , a laccase producing ascomycete recently isolated from soil , was studied to eliminate chlorophenol derivatives in submerged culture medium .
	manualset3
155069	2	408485	13	NULL	NULL	0	NULL	Paraconiothyrium variabile	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of Paraconiothyrium variabile , a laccase producing ascomycete recently isolated from soil , was studied to eliminate chlorophenol derivatives in submerged culture medium .
	manualset3
155070	3	408485	13	NULL	NULL	0	NULL	laccase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of Paraconiothyrium variabile , a laccase producing ascomycete recently isolated from soil , was studied to eliminate chlorophenol derivatives in submerged culture medium .
	manualset3
155071	4	408485	13	NULL	NULL	0	NULL	ascomycete	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of Paraconiothyrium variabile , a laccase producing ascomycete recently isolated from soil , was studied to eliminate chlorophenol derivatives in submerged culture medium .
	manualset3
155072	5	408485	13	NULL	NULL	0	NULL	soil	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of Paraconiothyrium variabile , a laccase producing ascomycete recently isolated from soil , was studied to eliminate chlorophenol derivatives in submerged culture medium .
	manualset3
155073	6	408485	13	NULL	NULL	0	NULL	chlorophenol derivatives	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of Paraconiothyrium variabile , a laccase producing ascomycete recently isolated from soil , was studied to eliminate chlorophenol derivatives in submerged culture medium .
	manualset3
155074	7	408485	13	NULL	NULL	0	NULL	culture medium	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of Paraconiothyrium variabile , a laccase producing ascomycete recently isolated from soil , was studied to eliminate chlorophenol derivatives in submerged culture medium .
	manualset3
155075	1	408486	13	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of `` fluid , '' haptenated liposomes specifically to stimulate or to suppress the TI PFC response is determined by the ratio of hapten to other lipids in a manner that is independent of the total hapten concentration in culture .
	manualset3
155076	2	408486	13	NULL	NULL	0	NULL	fluid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of `` fluid , '' haptenated liposomes specifically to stimulate or to suppress the TI PFC response is determined by the ratio of hapten to other lipids in a manner that is independent of the total hapten concentration in culture .
	manualset3
155077	3	408486	13	NULL	NULL	0	NULL	liposomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of `` fluid , '' haptenated liposomes specifically to stimulate or to suppress the TI PFC response is determined by the ratio of hapten to other lipids in a manner that is independent of the total hapten concentration in culture .
	manualset3
155078	4	408486	13	NULL	NULL	0	NULL	TI PFC response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of `` fluid , '' haptenated liposomes specifically to stimulate or to suppress the TI PFC response is determined by the ratio of hapten to other lipids in a manner that is independent of the total hapten concentration in culture .
	manualset3
155079	5	408486	13	NULL	NULL	0	NULL	ratio of hapten	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of `` fluid , '' haptenated liposomes specifically to stimulate or to suppress the TI PFC response is determined by the ratio of hapten to other lipids in a manner that is independent of the total hapten concentration in culture .
	manualset3
155080	6	408486	13	NULL	NULL	0	NULL	lipids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of `` fluid , '' haptenated liposomes specifically to stimulate or to suppress the TI PFC response is determined by the ratio of hapten to other lipids in a manner that is independent of the total hapten concentration in culture .
	manualset3
155081	7	408486	13	NULL	NULL	0	NULL	manner	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of `` fluid , '' haptenated liposomes specifically to stimulate or to suppress the TI PFC response is determined by the ratio of hapten to other lipids in a manner that is independent of the total hapten concentration in culture .
	manualset3
155082	8	408486	13	NULL	NULL	0	NULL	hapten concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of `` fluid , '' haptenated liposomes specifically to stimulate or to suppress the TI PFC response is determined by the ratio of hapten to other lipids in a manner that is independent of the total hapten concentration in culture .
	manualset3
155083	9	408486	13	NULL	NULL	0	NULL	culture	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of `` fluid , '' haptenated liposomes specifically to stimulate or to suppress the TI PFC response is determined by the ratio of hapten to other lipids in a manner that is independent of the total hapten concentration in culture .
	manualset3
155084	1	408487	13	NULL	NULL	0	NULL	ability 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of insulin to increase cell number , stimulate bromodeoxyuridine incorporation and reduce caspase 3-like activity was prevented by PD98059 , which inhibits activation of the Drosophila extracellular signal regulated kinase ( DERK ) pathway , and was unaffected by wortmannin , an inhibitor of Drosophila phosphatidylinositol 3-kinase ( DPI3K ) .
	manualset3
155085	2	408487	13	NULL	NULL	0	NULL	insulin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of insulin to increase cell number , stimulate bromodeoxyuridine incorporation and reduce caspase 3-like activity was prevented by PD98059 , which inhibits activation of the Drosophila extracellular signal regulated kinase ( DERK ) pathway , and was unaffected by wortmannin , an inhibitor of Drosophila phosphatidylinositol 3-kinase ( DPI3K ) .
	manualset3
155086	3	408487	13	NULL	NULL	0	NULL	cell number	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of insulin to increase cell number , stimulate bromodeoxyuridine incorporation and reduce caspase 3-like activity was prevented by PD98059 , which inhibits activation of the Drosophila extracellular signal regulated kinase ( DERK ) pathway , and was unaffected by wortmannin , an inhibitor of Drosophila phosphatidylinositol 3-kinase ( DPI3K ) .
	manualset3
155087	4	408487	13	NULL	NULL	0	NULL	bromodeoxyuridine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of insulin to increase cell number , stimulate bromodeoxyuridine incorporation and reduce caspase 3-like activity was prevented by PD98059 , which inhibits activation of the Drosophila extracellular signal regulated kinase ( DERK ) pathway , and was unaffected by wortmannin , an inhibitor of Drosophila phosphatidylinositol 3-kinase ( DPI3K ) .
	manualset3
155088	5	408487	13	NULL	NULL	0	NULL	incorporation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of insulin to increase cell number , stimulate bromodeoxyuridine incorporation and reduce caspase 3-like activity was prevented by PD98059 , which inhibits activation of the Drosophila extracellular signal regulated kinase ( DERK ) pathway , and was unaffected by wortmannin , an inhibitor of Drosophila phosphatidylinositol 3-kinase ( DPI3K ) .
	manualset3
155090	6	408487	13	NULL	NULL	NULL	NULL	caspase 3-like activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ability of insulin to increase cell number , stimulate bromodeoxyuridine incorporation and reduce caspase 3-like activity was prevented by PD98059 , which inhibits activation of the Drosophila extracellular signal regulated kinase ( DERK ) pathway , and was unaffected by wortmannin , an inhibitor of Drosophila phosphatidylinositol 3-kinase ( DPI3K ) .
	manualset3
155091	7	408487	13	NULL	NULL	0	NULL	PD98059	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of insulin to increase cell number , stimulate bromodeoxyuridine incorporation and reduce caspase 3-like activity was prevented by PD98059 , which inhibits activation of the Drosophila extracellular signal regulated kinase ( DERK ) pathway , and was unaffected by wortmannin , an inhibitor of Drosophila phosphatidylinositol 3-kinase ( DPI3K ) .
	manualset3
155092	8	408487	13	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of insulin to increase cell number , stimulate bromodeoxyuridine incorporation and reduce caspase 3-like activity was prevented by PD98059 , which inhibits activation of the Drosophila extracellular signal regulated kinase ( DERK ) pathway , and was unaffected by wortmannin , an inhibitor of Drosophila phosphatidylinositol 3-kinase ( DPI3K ) .
	manualset3
155093	9	408487	13	NULL	NULL	0	NULL	Drosophila extracellular signal regulated kinase ( DERK ) pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of insulin to increase cell number , stimulate bromodeoxyuridine incorporation and reduce caspase 3-like activity was prevented by PD98059 , which inhibits activation of the Drosophila extracellular signal regulated kinase ( DERK ) pathway , and was unaffected by wortmannin , an inhibitor of Drosophila phosphatidylinositol 3-kinase ( DPI3K ) .
	manualset3
155094	10	408487	13	NULL	NULL	0	NULL	wortmannin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of insulin to increase cell number , stimulate bromodeoxyuridine incorporation and reduce caspase 3-like activity was prevented by PD98059 , which inhibits activation of the Drosophila extracellular signal regulated kinase ( DERK ) pathway , and was unaffected by wortmannin , an inhibitor of Drosophila phosphatidylinositol 3-kinase ( DPI3K ) .
	manualset3
155095	11	408487	13	NULL	NULL	0	NULL	inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of insulin to increase cell number , stimulate bromodeoxyuridine incorporation and reduce caspase 3-like activity was prevented by PD98059 , which inhibits activation of the Drosophila extracellular signal regulated kinase ( DERK ) pathway , and was unaffected by wortmannin , an inhibitor of Drosophila phosphatidylinositol 3-kinase ( DPI3K ) .
	manualset3
155096	12	408487	13	NULL	NULL	0	NULL	Drosophila phosphatidylinositol 3-kinase ( DPI3K ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of insulin to increase cell number , stimulate bromodeoxyuridine incorporation and reduce caspase 3-like activity was prevented by PD98059 , which inhibits activation of the Drosophila extracellular signal regulated kinase ( DERK ) pathway , and was unaffected by wortmannin , an inhibitor of Drosophila phosphatidylinositol 3-kinase ( DPI3K ) .
	manualset3
155097	1	408488	13	NULL	NULL	0	NULL	ability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of mutant p53 143Val to Ala to inactivate the HPV early promoter in normal cells ( by approximately 60 % reduction ) suggests that this mutant may be able to associate with wild-type p53 and interact with TATA box-binding proteins .
	manualset3
155098	2	408488	13	NULL	NULL	0	NULL	mutant p53 143Val to Ala	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of mutant p53 143Val to Ala to inactivate the HPV early promoter in normal cells ( by approximately 60 % reduction ) suggests that this mutant may be able to associate with wild-type p53 and interact with TATA box-binding proteins .
	manualset3
155099	3	408488	13	NULL	NULL	0	NULL	HPV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of mutant p53 143Val to Ala to inactivate the HPV early promoter in normal cells ( by approximately 60 % reduction ) suggests that this mutant may be able to associate with wild-type p53 and interact with TATA box-binding proteins .
	manualset3
155100	4	408488	13	NULL	NULL	0	NULL	promoter 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of mutant p53 143Val to Ala to inactivate the HPV early promoter in normal cells ( by approximately 60 % reduction ) suggests that this mutant may be able to associate with wild-type p53 and interact with TATA box-binding proteins .
	manualset3
155101	5	408488	13	NULL	NULL	0	NULL	normal cells	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of mutant p53 143Val to Ala to inactivate the HPV early promoter in normal cells ( by approximately 60 % reduction ) suggests that this mutant may be able to associate with wild-type p53 and interact with TATA box-binding proteins .
	manualset3
155102	6	408488	13	NULL	NULL	0	NULL	approximately 60 % reduction	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of mutant p53 143Val to Ala to inactivate the HPV early promoter in normal cells ( by approximately 60 % reduction ) suggests that this mutant may be able to associate with wild-type p53 and interact with TATA box-binding proteins .
	manualset3
155103	7	408488	13	NULL	NULL	0	NULL	mutant 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of mutant p53 143Val to Ala to inactivate the HPV early promoter in normal cells ( by approximately 60 % reduction ) suggests that this mutant may be able to associate with wild-type p53 and interact with TATA box-binding proteins .
	manualset3
155104	8	408488	13	NULL	NULL	0	NULL	wild-type p53	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of mutant p53 143Val to Ala to inactivate the HPV early promoter in normal cells ( by approximately 60 % reduction ) suggests that this mutant may be able to associate with wild-type p53 and interact with TATA box-binding proteins .
	manualset3
155105	9	408488	13	NULL	NULL	0	NULL	TATA box-binding proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of mutant p53 143Val to Ala to inactivate the HPV early promoter in normal cells ( by approximately 60 % reduction ) suggests that this mutant may be able to associate with wild-type p53 and interact with TATA box-binding proteins .
	manualset3
155106	1	408489	13	NULL	NULL	0	NULL	ability 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of splenocytes to generate an Ab response to SRBC was significantly elevated following treatment regime A and at the lower dose in treatment regime D. All other treatment protocols did not alter this immune parameter .
	manualset3
155107	2	408489	13	NULL	NULL	0	NULL	splenocytes	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of splenocytes to generate an Ab response to SRBC was significantly elevated following treatment regime A and at the lower dose in treatment regime D. All other treatment protocols did not alter this immune parameter .
	manualset3
155108	3	408489	13	NULL	NULL	0	NULL	Ab response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of splenocytes to generate an Ab response to SRBC was significantly elevated following treatment regime A and at the lower dose in treatment regime D. All other treatment protocols did not alter this immune parameter .
	manualset3
155109	4	408489	13	NULL	NULL	0	NULL	SRBC 	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of splenocytes to generate an Ab response to SRBC was significantly elevated following treatment regime A and at the lower dose in treatment regime D. All other treatment protocols did not alter this immune parameter .
	manualset3
155110	5	408489	13	NULL	NULL	0	NULL	treatment regime A	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of splenocytes to generate an Ab response to SRBC was significantly elevated following treatment regime A and at the lower dose in treatment regime D. All other treatment protocols did not alter this immune parameter .
	manualset3
155111	6	408489	13	NULL	NULL	0	NULL	dose	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of splenocytes to generate an Ab response to SRBC was significantly elevated following treatment regime A and at the lower dose in treatment regime D. All other treatment protocols did not alter this immune parameter .
	manualset3
155112	7	408489	13	NULL	NULL	0	NULL	treatment regime D	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of splenocytes to generate an Ab response to SRBC was significantly elevated following treatment regime A and at the lower dose in treatment regime D. All other treatment protocols did not alter this immune parameter .
	manualset3
155113	8	408489	13	NULL	NULL	0	NULL	treatment protocols	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of splenocytes to generate an Ab response to SRBC was significantly elevated following treatment regime A and at the lower dose in treatment regime D. All other treatment protocols did not alter this immune parameter .
	manualset3
155114	9	408489	13	NULL	NULL	0	NULL	immune parameter	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of splenocytes to generate an Ab response to SRBC was significantly elevated following treatment regime A and at the lower dose in treatment regime D. All other treatment protocols did not alter this immune parameter .
	manualset3
155115	1	408490	13	NULL	NULL	0	NULL	ability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of the TMT to accurately assess fall risk was determined using validity index measures .
	manualset3
155116	2	408490	13	NULL	NULL	0	NULL	TMT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of the TMT to accurately assess fall risk was determined using validity index measures .
	manualset3
155117	3	408490	13	NULL	NULL	0	NULL	fall risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of the TMT to accurately assess fall risk was determined using validity index measures .
	manualset3
155118	4	408490	13	NULL	NULL	0	NULL	validity index measures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of the TMT to accurately assess fall risk was determined using validity index measures .
	manualset3
155119	1	408491	13	NULL	NULL	0	NULL	ability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of the enzyme to cleave other proteins , including kininogen and transferrin , suggests that it has specificity for the Pro-X-Gly sequence found in several proteins , including collagen .
	manualset3
155120	2	408491	13	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of the enzyme to cleave other proteins , including kininogen and transferrin , suggests that it has specificity for the Pro-X-Gly sequence found in several proteins , including collagen .
	manualset3
155121	3	408491	13	NULL	NULL	0	NULL	proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of the enzyme to cleave other proteins , including kininogen and transferrin , suggests that it has specificity for the Pro-X-Gly sequence found in several proteins , including collagen .
	manualset3
155122	4	408491	13	NULL	NULL	0	NULL	kininogen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of the enzyme to cleave other proteins , including kininogen and transferrin , suggests that it has specificity for the Pro-X-Gly sequence found in several proteins , including collagen .
	manualset3
155123	5	408491	13	NULL	NULL	0	NULL	transferrin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of the enzyme to cleave other proteins , including kininogen and transferrin , suggests that it has specificity for the Pro-X-Gly sequence found in several proteins , including collagen .
	manualset3
155124	6	408491	13	NULL	NULL	0	NULL	specificity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of the enzyme to cleave other proteins , including kininogen and transferrin , suggests that it has specificity for the Pro-X-Gly sequence found in several proteins , including collagen .
	manualset3
155125	7	408491	13	NULL	NULL	0	NULL	Pro-X-Gly sequence	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of the enzyme to cleave other proteins , including kininogen and transferrin , suggests that it has specificity for the Pro-X-Gly sequence found in several proteins , including collagen .
	manualset3
155126	8	408491	13	NULL	NULL	0	NULL	several proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of the enzyme to cleave other proteins , including kininogen and transferrin , suggests that it has specificity for the Pro-X-Gly sequence found in several proteins , including collagen .
	manualset3
155127	9	408491	13	NULL	NULL	0	NULL	collagen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of the enzyme to cleave other proteins , including kininogen and transferrin , suggests that it has specificity for the Pro-X-Gly sequence found in several proteins , including collagen .
	manualset3
155128	1	408492	13	NULL	NULL	0	NULL	ability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of the human luteal cell to respond to hCG with cAMP accumulation and the ability of adenosine to amplify this cAMP response appeared to be inversely related to human luteal cell age .
	manualset3
155129	2	408492	13	NULL	NULL	0	NULL	human luteal cell 	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of the human luteal cell to respond to hCG with cAMP accumulation and the ability of adenosine to amplify this cAMP response appeared to be inversely related to human luteal cell age .
	manualset3
155130	3	408492	13	NULL	NULL	0	NULL	hCG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of the human luteal cell to respond to hCG with cAMP accumulation and the ability of adenosine to amplify this cAMP response appeared to be inversely related to human luteal cell age .
	manualset3
155131	4	408492	13	NULL	NULL	0	NULL	cAMP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of the human luteal cell to respond to hCG with cAMP accumulation and the ability of adenosine to amplify this cAMP response appeared to be inversely related to human luteal cell age .
	manualset3
155132	5	408492	13	NULL	NULL	0	NULL	accumulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of the human luteal cell to respond to hCG with cAMP accumulation and the ability of adenosine to amplify this cAMP response appeared to be inversely related to human luteal cell age .
	manualset3
155133	6	408492	13	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of the human luteal cell to respond to hCG with cAMP accumulation and the ability of adenosine to amplify this cAMP response appeared to be inversely related to human luteal cell age .
	manualset3
155134	7	408492	13	NULL	NULL	0	NULL	adenosine	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of the human luteal cell to respond to hCG with cAMP accumulation and the ability of adenosine to amplify this cAMP response appeared to be inversely related to human luteal cell age .
	manualset3
155135	8	408492	13	NULL	NULL	0	NULL	cAMP response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of the human luteal cell to respond to hCG with cAMP accumulation and the ability of adenosine to amplify this cAMP response appeared to be inversely related to human luteal cell age .
	manualset3
155136	9	408492	13	NULL	NULL	0	NULL	human luteal cell 	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of the human luteal cell to respond to hCG with cAMP accumulation and the ability of adenosine to amplify this cAMP response appeared to be inversely related to human luteal cell age .
	manualset3
155137	10	408492	13	NULL	NULL	0	NULL	age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of the human luteal cell to respond to hCG with cAMP accumulation and the ability of adenosine to amplify this cAMP response appeared to be inversely related to human luteal cell age .
	manualset3
155138	1	408493	13	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability to deliver IMRT fields wider than 14.5 cm with the Millennium MLC has improved the efficiency and flexibility of IMRT treatments ; however , significant extra dose can be introduced due to end leaf leakage .
	manualset3
155139	2	408493	13	NULL	NULL	0	NULL	IMRT fields	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability to deliver IMRT fields wider than 14.5 cm with the Millennium MLC has improved the efficiency and flexibility of IMRT treatments ; however , significant extra dose can be introduced due to end leaf leakage .
	manualset3
155140	3	408493	13	NULL	NULL	0	NULL	14.5 cm 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability to deliver IMRT fields wider than 14.5 cm with the Millennium MLC has improved the efficiency and flexibility of IMRT treatments ; however , significant extra dose can be introduced due to end leaf leakage .
	manualset3
155141	4	408493	13	NULL	NULL	0	NULL	Millennium MLC 	thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability to deliver IMRT fields wider than 14.5 cm with the Millennium MLC has improved the efficiency and flexibility of IMRT treatments ; however , significant extra dose can be introduced due to end leaf leakage .
	manualset3
155142	5	408493	13	NULL	NULL	0	NULL	efficiency	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability to deliver IMRT fields wider than 14.5 cm with the Millennium MLC has improved the efficiency and flexibility of IMRT treatments ; however , significant extra dose can be introduced due to end leaf leakage .
	manualset3
155143	6	408493	13	NULL	NULL	0	NULL	flexibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability to deliver IMRT fields wider than 14.5 cm with the Millennium MLC has improved the efficiency and flexibility of IMRT treatments ; however , significant extra dose can be introduced due to end leaf leakage .
	manualset3
155144	7	408493	13	NULL	NULL	0	NULL	IMRT treatments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability to deliver IMRT fields wider than 14.5 cm with the Millennium MLC has improved the efficiency and flexibility of IMRT treatments ; however , significant extra dose can be introduced due to end leaf leakage .
	manualset3
155145	8	408493	13	NULL	NULL	0	NULL	dose	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability to deliver IMRT fields wider than 14.5 cm with the Millennium MLC has improved the efficiency and flexibility of IMRT treatments ; however , significant extra dose can be introduced due to end leaf leakage .
	manualset3
155146	9	408493	13	NULL	NULL	0	NULL	leaf leakage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability to deliver IMRT fields wider than 14.5 cm with the Millennium MLC has improved the efficiency and flexibility of IMRT treatments ; however , significant extra dose can be introduced due to end leaf leakage .
	manualset3
155147	1	408494	13	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability to induce specific regulation or removal of autoreactive T cells will allow for the first time an assessment of cause and effect in human diseases .
	manualset3
155148	2	408494	13	NULL	NULL	0	NULL	regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability to induce specific regulation or removal of autoreactive T cells will allow for the first time an assessment of cause and effect in human diseases .
	manualset3
155149	3	408494	13	NULL	NULL	0	NULL	removal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability to induce specific regulation or removal of autoreactive T cells will allow for the first time an assessment of cause and effect in human diseases .
	manualset3
155150	4	408494	13	NULL	NULL	0	NULL	autoreactive T cells	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability to induce specific regulation or removal of autoreactive T cells will allow for the first time an assessment of cause and effect in human diseases .
	manualset3
155151	5	408494	13	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability to induce specific regulation or removal of autoreactive T cells will allow for the first time an assessment of cause and effect in human diseases .
	manualset3
155152	6	408494	13	NULL	NULL	0	NULL	assessment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability to induce specific regulation or removal of autoreactive T cells will allow for the first time an assessment of cause and effect in human diseases .
	manualset3
155153	7	408494	13	NULL	NULL	0	NULL	cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability to induce specific regulation or removal of autoreactive T cells will allow for the first time an assessment of cause and effect in human diseases .
	manualset3
155154	8	408494	13	NULL	NULL	0	NULL	effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability to induce specific regulation or removal of autoreactive T cells will allow for the first time an assessment of cause and effect in human diseases .
	manualset3
155155	9	408494	13	NULL	NULL	0	NULL	human diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability to induce specific regulation or removal of autoreactive T cells will allow for the first time an assessment of cause and effect in human diseases .
	manualset3
155174	1	408495	13	NULL	NULL	0	NULL	 abnormal macula densa ultrastructure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The abnormal macula densa ultrastructure has been suggested to be connected with the functional abnormalities in diabetes , i.e. the resetting of the tubuloglomerular feedback and subsequent increases in GFR .
	manualset3
155175	2	408495	13	NULL	NULL	0	NULL	functional abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The abnormal macula densa ultrastructure has been suggested to be connected with the functional abnormalities in diabetes , i.e. the resetting of the tubuloglomerular feedback and subsequent increases in GFR .
	manualset3
155176	3	408495	13	NULL	NULL	0	NULL	diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The abnormal macula densa ultrastructure has been suggested to be connected with the functional abnormalities in diabetes , i.e. the resetting of the tubuloglomerular feedback and subsequent increases in GFR .
	manualset3
155177	4	408495	13	NULL	NULL	0	NULL	tubuloglomerular feedback 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The abnormal macula densa ultrastructure has been suggested to be connected with the functional abnormalities in diabetes , i.e. the resetting of the tubuloglomerular feedback and subsequent increases in GFR .
	manualset3
155178	5	408495	13	NULL	NULL	0	NULL	increases	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The abnormal macula densa ultrastructure has been suggested to be connected with the functional abnormalities in diabetes , i.e. the resetting of the tubuloglomerular feedback and subsequent increases in GFR .
	manualset3
155179	6	408495	13	NULL	NULL	0	NULL	GFR	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The abnormal macula densa ultrastructure has been suggested to be connected with the functional abnormalities in diabetes , i.e. the resetting of the tubuloglomerular feedback and subsequent increases in GFR .
	manualset3
155180	1	408496	13	NULL	NULL	0	NULL	abnormalities 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The abnormalities consisted of VSD ( 7 patients ) and moderate aortic regurgitation ( 2 ) .
	manualset3
155181	2	408496	13	NULL	NULL	0	NULL	 VSD	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The abnormalities consisted of VSD ( 7 patients ) and moderate aortic regurgitation ( 2 ) .
	manualset3
155182	3	408496	13	NULL	NULL	0	NULL	7 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The abnormalities consisted of VSD ( 7 patients ) and moderate aortic regurgitation ( 2 ) .
	manualset3
155183	4	408496	13	NULL	NULL	0	NULL	moderate aortic regurgitation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The abnormalities consisted of VSD ( 7 patients ) and moderate aortic regurgitation ( 2 ) .
	manualset3
155184	1	408497	13	NULL	NULL	0	NULL	74 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The about 74 % inactivation of the enzymic activity on covalent pyridoxal-P treatment of the FMO was nearly completely prevented in the presence of the substrate , N , N-dimethylaniline .
	manualset3
155185	2	408497	13	NULL	NULL	0	NULL	inactivation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The about 74 % inactivation of the enzymic activity on covalent pyridoxal-P treatment of the FMO was nearly completely prevented in the presence of the substrate , N , N-dimethylaniline .
	manualset3
155186	3	408497	13	NULL	NULL	0	NULL	enzymic activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The about 74 % inactivation of the enzymic activity on covalent pyridoxal-P treatment of the FMO was nearly completely prevented in the presence of the substrate , N , N-dimethylaniline .
	manualset3
155187	4	408497	13	NULL	NULL	0	NULL	covalent pyridoxal-P treatment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The about 74 % inactivation of the enzymic activity on covalent pyridoxal-P treatment of the FMO was nearly completely prevented in the presence of the substrate , N , N-dimethylaniline .
	manualset3
155188	5	408497	13	NULL	NULL	0	NULL	FMO	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The about 74 % inactivation of the enzymic activity on covalent pyridoxal-P treatment of the FMO was nearly completely prevented in the presence of the substrate , N , N-dimethylaniline .
	manualset3
155189	6	408497	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The about 74 % inactivation of the enzymic activity on covalent pyridoxal-P treatment of the FMO was nearly completely prevented in the presence of the substrate , N , N-dimethylaniline .
	manualset3
155190	7	408497	13	NULL	NULL	0	NULL	 substrate , N , N-dimethylaniline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The about 74 % inactivation of the enzymic activity on covalent pyridoxal-P treatment of the FMO was nearly completely prevented in the presence of the substrate , N , N-dimethylaniline .
	manualset3
155191	1	408498	13	NULL	NULL	0	NULL	analogs	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The above analogs were shown to possess different affinities toward opiate receptors of mu-type .
	manualset3
155192	2	408498	13	NULL	NULL	0	NULL	affinities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The above analogs were shown to possess different affinities toward opiate receptors of mu-type .
	manualset3
155193	3	408498	13	NULL	NULL	0	NULL	opiate receptors of mu-type	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The above analogs were shown to possess different affinities toward opiate receptors of mu-type .
	manualset3
155194	1	408499	13	NULL	NULL	0	NULL	electrophysiological findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The above electrophysiological findings suggest that myoclonus following methyl bromide poisoning belongs to the cortical reflex myoclonus category .
	manualset3
155195	2	408499	13	NULL	NULL	0	NULL	myoclonus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The above electrophysiological findings suggest that myoclonus following methyl bromide poisoning belongs to the cortical reflex myoclonus category .
	manualset3
155196	3	408499	13	NULL	NULL	0	NULL	methyl bromide 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The above electrophysiological findings suggest that myoclonus following methyl bromide poisoning belongs to the cortical reflex myoclonus category .
	manualset3
155197	4	408499	13	NULL	NULL	0	NULL	cortical reflex myoclonus category 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The above electrophysiological findings suggest that myoclonus following methyl bromide poisoning belongs to the cortical reflex myoclonus category .
	manualset3
155198	1	408500	13	NULL	NULL	0	NULL	replicase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A replicase containing nsP1 , P23 , and nsP4 can make both plus and minus strands , but prefers the promoter for genomic plus sense RNA to that for subgenomic mRNA .
	manualset3
155199	2	408500	13	NULL	NULL	0	NULL	nsP1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A replicase containing nsP1 , P23 , and nsP4 can make both plus and minus strands , but prefers the promoter for genomic plus sense RNA to that for subgenomic mRNA .
	manualset3
155200	3	408500	13	NULL	NULL	0	NULL	P23	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A replicase containing nsP1 , P23 , and nsP4 can make both plus and minus strands , but prefers the promoter for genomic plus sense RNA to that for subgenomic mRNA .
	manualset3
155201	4	408500	13	NULL	NULL	0	NULL	nsP4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A replicase containing nsP1 , P23 , and nsP4 can make both plus and minus strands , but prefers the promoter for genomic plus sense RNA to that for subgenomic mRNA .
	manualset3
155202	5	408500	13	NULL	NULL	0	NULL	strands	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A replicase containing nsP1 , P23 , and nsP4 can make both plus and minus strands , but prefers the promoter for genomic plus sense RNA to that for subgenomic mRNA .
	manualset3
155203	6	408500	13	NULL	NULL	0	NULL	promoter 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A replicase containing nsP1 , P23 , and nsP4 can make both plus and minus strands , but prefers the promoter for genomic plus sense RNA to that for subgenomic mRNA .
	manualset3
155204	7	408500	13	NULL	NULL	0	NULL	genomic plus sense RNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A replicase containing nsP1 , P23 , and nsP4 can make both plus and minus strands , but prefers the promoter for genomic plus sense RNA to that for subgenomic mRNA .
	manualset3
155205	8	408500	13	NULL	NULL	0	NULL	subgenomic mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A replicase containing nsP1 , P23 , and nsP4 can make both plus and minus strands , but prefers the promoter for genomic plus sense RNA to that for subgenomic mRNA .
	manualset3
155206	1	408501	13	NULL	NULL	0	NULL	findings 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The above findings emphasise the importance of teleconsultation as a means to provide wide medical coverage within the region .
	manualset3
155207	2	408501	13	NULL	NULL	0	NULL	importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The above findings emphasise the importance of teleconsultation as a means to provide wide medical coverage within the region .
	manualset3
155208	3	408501	13	NULL	NULL	0	NULL	teleconsultation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The above findings emphasise the importance of teleconsultation as a means to provide wide medical coverage within the region .
	manualset3
155209	4	408501	13	NULL	NULL	0	NULL	means 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The above findings emphasise the importance of teleconsultation as a means to provide wide medical coverage within the region .
	manualset3
155210	5	408501	13	NULL	NULL	NULL	NULL	medical coverage	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The above findings emphasise the importance of teleconsultation as a means to provide wide medical coverage within the region .
	manualset3
155211	6	408501	13	NULL	NULL	0	NULL	region	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The above findings emphasise the importance of teleconsultation as a means to provide wide medical coverage within the region .
	manualset3
155212	1	408502	13	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The above results indicate that despite their similar in vivo anticarcinogenic effects , genistein and resveratrol appear to exert different effects on oxidative DNA damage in vitro .
	manualset3
155213	2	408502	13	NULL	NULL	0	NULL	anticarcinogenic effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The above results indicate that despite their similar in vivo anticarcinogenic effects , genistein and resveratrol appear to exert different effects on oxidative DNA damage in vitro .
	manualset3
155214	3	408502	13	NULL	NULL	0	NULL	genistein 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The above results indicate that despite their similar in vivo anticarcinogenic effects , genistein and resveratrol appear to exert different effects on oxidative DNA damage in vitro .
	manualset3
155215	4	408502	13	NULL	NULL	0	NULL	resveratrol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The above results indicate that despite their similar in vivo anticarcinogenic effects , genistein and resveratrol appear to exert different effects on oxidative DNA damage in vitro .
	manualset3
155216	5	408502	13	NULL	NULL	0	NULL	effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The above results indicate that despite their similar in vivo anticarcinogenic effects , genistein and resveratrol appear to exert different effects on oxidative DNA damage in vitro .
	manualset3
155217	6	408502	13	NULL	NULL	0	NULL	oxidative DNA damage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The above results indicate that despite their similar in vivo anticarcinogenic effects , genistein and resveratrol appear to exert different effects on oxidative DNA damage in vitro .
	manualset3
155223	1	408503	13	NULL	NULL	0	NULL	pig farming	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The abrupt weaning in pig farming comprises multiple stressful events such as change in diet , new physical environment , as well as the often underestimated psychosocial consequences of maternal deprivation and regrouping with unfamiliar conspecifics .
	manualset3
155225	2	408503	13	NULL	NULL	0	NULL	events	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The abrupt weaning in pig farming comprises multiple stressful events such as change in diet , new physical environment , as well as the often underestimated psychosocial consequences of maternal deprivation and regrouping with unfamiliar conspecifics .
	manualset3
155227	3	408503	13	NULL	NULL	0	NULL	change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The abrupt weaning in pig farming comprises multiple stressful events such as change in diet , new physical environment , as well as the often underestimated psychosocial consequences of maternal deprivation and regrouping with unfamiliar conspecifics .
	manualset3
155228	4	408503	13	NULL	NULL	0	NULL	diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The abrupt weaning in pig farming comprises multiple stressful events such as change in diet , new physical environment , as well as the often underestimated psychosocial consequences of maternal deprivation and regrouping with unfamiliar conspecifics .
	manualset3
155230	5	408503	13	NULL	NULL	0	NULL	physical environment	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The abrupt weaning in pig farming comprises multiple stressful events such as change in diet , new physical environment , as well as the often underestimated psychosocial consequences of maternal deprivation and regrouping with unfamiliar conspecifics .
	manualset3
155231	6	408503	13	NULL	NULL	0	NULL	psychosocial consequences 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The abrupt weaning in pig farming comprises multiple stressful events such as change in diet , new physical environment , as well as the often underestimated psychosocial consequences of maternal deprivation and regrouping with unfamiliar conspecifics .
	manualset3
155232	7	408503	13	NULL	NULL	0	NULL	deprivation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The abrupt weaning in pig farming comprises multiple stressful events such as change in diet , new physical environment , as well as the often underestimated psychosocial consequences of maternal deprivation and regrouping with unfamiliar conspecifics .
	manualset3
155233	8	408503	13	NULL	NULL	0	NULL	regrouping	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The abrupt weaning in pig farming comprises multiple stressful events such as change in diet , new physical environment , as well as the often underestimated psychosocial consequences of maternal deprivation and regrouping with unfamiliar conspecifics .
	manualset3
155234	9	408503	13	NULL	NULL	0	NULL	conspecifics	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The abrupt weaning in pig farming comprises multiple stressful events such as change in diet , new physical environment , as well as the often underestimated psychosocial consequences of maternal deprivation and regrouping with unfamiliar conspecifics .
	manualset3
155235	1	408504	13	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of CA joint ankylosis permits the efficacy of thyroplasty medialization procedures .
	manualset3
155236	2	408504	13	NULL	NULL	0	NULL	CA joint ankylosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of CA joint ankylosis permits the efficacy of thyroplasty medialization procedures .
	manualset3
155237	3	408504	13	NULL	NULL	0	NULL	efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of CA joint ankylosis permits the efficacy of thyroplasty medialization procedures .
	manualset3
155238	4	408504	13	NULL	NULL	0	NULL	thyroplasty medialization procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of CA joint ankylosis permits the efficacy of thyroplasty medialization procedures .
	manualset3
155242	1	408505	13	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of COX-1 or COX-2 did not appear to effect ocular development in these mice .
	manualset3
155243	2	408505	13	NULL	NULL	0	NULL	COX-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of COX-1 or COX-2 did not appear to effect ocular development in these mice .
	manualset3
155244	3	408505	13	NULL	NULL	0	NULL	COX-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of COX-1 or COX-2 did not appear to effect ocular development in these mice .
	manualset3
155245	4	408505	13	NULL	NULL	0	NULL	ocular development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of COX-1 or COX-2 did not appear to effect ocular development in these mice .
	manualset3
155247	5	408505	13	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of COX-1 or COX-2 did not appear to effect ocular development in these mice .
	manualset3
155249	1	408506	13	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of apoptotic death correlates with a specific defect in activation of Bax .
	manualset3
155250	2	408506	13	NULL	NULL	0	NULL	apoptotic death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of apoptotic death correlates with a specific defect in activation of Bax .
	manualset3
155251	3	408506	13	NULL	NULL	0	NULL	defect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of apoptotic death correlates with a specific defect in activation of Bax .
	manualset3
155252	4	408506	13	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of apoptotic death correlates with a specific defect in activation of Bax .
	manualset3
155254	5	408506	13	NULL	NULL	0	NULL	Bax	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of apoptotic death correlates with a specific defect in activation of Bax .
	manualset3
155261	1	408507	13	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of axial loading and lumbar extension results in a maximization of spinal canal dimensions , which may in some cases , result in failure to demonstrate nerve root compression .
	manualset3
155263	2	408507	13	NULL	NULL	0	NULL	axial loading	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of axial loading and lumbar extension results in a maximization of spinal canal dimensions , which may in some cases , result in failure to demonstrate nerve root compression .
	manualset3
155264	3	408507	13	NULL	NULL	0	NULL	lumbar extension results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of axial loading and lumbar extension results in a maximization of spinal canal dimensions , which may in some cases , result in failure to demonstrate nerve root compression .
	manualset3
155265	4	408507	13	NULL	NULL	0	NULL	maximization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of axial loading and lumbar extension results in a maximization of spinal canal dimensions , which may in some cases , result in failure to demonstrate nerve root compression .
	manualset3
155266	5	408507	13	NULL	NULL	0	NULL	spinal canal dimensions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of axial loading and lumbar extension results in a maximization of spinal canal dimensions , which may in some cases , result in failure to demonstrate nerve root compression .
	manualset3
155267	6	408507	13	NULL	NULL	0	NULL	cases 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of axial loading and lumbar extension results in a maximization of spinal canal dimensions , which may in some cases , result in failure to demonstrate nerve root compression .
	manualset3
155268	7	408507	13	NULL	NULL	0	NULL	result	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of axial loading and lumbar extension results in a maximization of spinal canal dimensions , which may in some cases , result in failure to demonstrate nerve root compression .
	manualset3
155269	8	408507	13	NULL	NULL	0	NULL	failure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of axial loading and lumbar extension results in a maximization of spinal canal dimensions , which may in some cases , result in failure to demonstrate nerve root compression .
	manualset3
155270	9	408507	13	NULL	NULL	0	NULL	nerve root compression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of axial loading and lumbar extension results in a maximization of spinal canal dimensions , which may in some cases , result in failure to demonstrate nerve root compression .
	manualset3
155271	1	408508	13	NULL	NULL	0	NULL	absence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of deconjugated bile acids in the duodenal juice of most infants with protracted diarrhoea suggests that they do not contribute significantly to the pathophysiology of this disorder .
	manualset3
155272	2	408508	13	NULL	NULL	0	NULL	bile acids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of deconjugated bile acids in the duodenal juice of most infants with protracted diarrhoea suggests that they do not contribute significantly to the pathophysiology of this disorder .
	manualset3
155273	3	408508	13	NULL	NULL	0	NULL	duodenal juice	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of deconjugated bile acids in the duodenal juice of most infants with protracted diarrhoea suggests that they do not contribute significantly to the pathophysiology of this disorder .
	manualset3
155274	4	408508	13	NULL	NULL	0	NULL	infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of deconjugated bile acids in the duodenal juice of most infants with protracted diarrhoea suggests that they do not contribute significantly to the pathophysiology of this disorder .
	manualset3
155275	5	408508	13	NULL	NULL	0	NULL	diarrhoea	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of deconjugated bile acids in the duodenal juice of most infants with protracted diarrhoea suggests that they do not contribute significantly to the pathophysiology of this disorder .
	manualset3
155276	6	408508	13	NULL	NULL	0	NULL	pathophysiology 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of deconjugated bile acids in the duodenal juice of most infants with protracted diarrhoea suggests that they do not contribute significantly to the pathophysiology of this disorder .
	manualset3
155277	7	408508	13	NULL	NULL	0	NULL	disorder	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of deconjugated bile acids in the duodenal juice of most infants with protracted diarrhoea suggests that they do not contribute significantly to the pathophysiology of this disorder .
	manualset3
155278	1	408509	13	NULL	NULL	0	NULL	absence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of reactivity was not linked with antibodies to salmozan or with some other serum factor .
	manualset3
155279	2	408509	13	NULL	NULL	0	NULL	reactivity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of reactivity was not linked with antibodies to salmozan or with some other serum factor .
	manualset3
155280	3	408509	13	NULL	NULL	0	NULL	antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The absence of reactivity was not linked with antibodies to salmozan or with some other serum factor .
	manualset3
155281	4	408509	13	NULL	NULL	NULL	NULL	salmozan	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The absence of reactivity was not linked with antibodies to salmozan or with some other serum factor .
	manualset3
155282	5	408509	13	NULL	NULL	NULL	NULL	serum factor	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The absence of reactivity was not linked with antibodies to salmozan or with some other serum factor .
	manualset3
155283	1	408510	13	NULL	NULL	NULL	NULL	 5-year survival rate	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The absolute 5-year survival rate was 67 % for the N0-N1 patients and 43 % for the N2-N3 patients .
	manualset3
155285	3	408510	13	NULL	NULL	0	NULL	67 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The absolute 5-year survival rate was 67 % for the N0-N1 patients and 43 % for the N2-N3 patients .
	manualset3
155286	4	408510	13	NULL	NULL	0	NULL	N0-N1 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The absolute 5-year survival rate was 67 % for the N0-N1 patients and 43 % for the N2-N3 patients .
	manualset3
155287	5	408510	13	NULL	NULL	NULL	NULL	43 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The absolute 5-year survival rate was 67 % for the N0-N1 patients and 43 % for the N2-N3 patients .
	manualset3
155288	6	408510	13	NULL	NULL	0	NULL	N2-N3 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The absolute 5-year survival rate was 67 % for the N0-N1 patients and 43 % for the N2-N3 patients .
	manualset3
155289	1	408511	13	NULL	NULL	0	NULL	requirement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The absolute requirement of pSC101 for dnaA in the integratively suppressed Hfr strain provides a useful system for further investigation of the dnaA function .
	manualset3
155290	2	408511	13	NULL	NULL	0	NULL	pSC101	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The absolute requirement of pSC101 for dnaA in the integratively suppressed Hfr strain provides a useful system for further investigation of the dnaA function .
	manualset3
155291	3	408511	13	NULL	NULL	0	NULL	dnaA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The absolute requirement of pSC101 for dnaA in the integratively suppressed Hfr strain provides a useful system for further investigation of the dnaA function .
	manualset3
155292	4	408511	13	NULL	NULL	0	NULL	Hfr strain	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The absolute requirement of pSC101 for dnaA in the integratively suppressed Hfr strain provides a useful system for further investigation of the dnaA function .
	manualset3
155293	5	408511	13	NULL	NULL	0	NULL	useful system	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The absolute requirement of pSC101 for dnaA in the integratively suppressed Hfr strain provides a useful system for further investigation of the dnaA function .
	manualset3
155294	6	408511	13	NULL	NULL	0	NULL	investigation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The absolute requirement of pSC101 for dnaA in the integratively suppressed Hfr strain provides a useful system for further investigation of the dnaA function .
	manualset3
155295	7	408511	13	NULL	NULL	0	NULL	dnaA function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The absolute requirement of pSC101 for dnaA in the integratively suppressed Hfr strain provides a useful system for further investigation of the dnaA function .
	manualset3
155296	1	408512	13	NULL	NULL	0	NULL	lipid	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorbed lipid was extracted from the disks with ether and analyzed for wax esters by thin-layer chromatography .
	manualset3
155297	2	408512	13	NULL	NULL	0	NULL	disks	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorbed lipid was extracted from the disks with ether and analyzed for wax esters by thin-layer chromatography .
	manualset3
155298	3	408512	13	NULL	NULL	0	NULL	ether	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorbed lipid was extracted from the disks with ether and analyzed for wax esters by thin-layer chromatography .
	manualset3
155299	4	408512	13	NULL	NULL	0	NULL	wax esters	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorbed lipid was extracted from the disks with ether and analyzed for wax esters by thin-layer chromatography .
	manualset3
155300	5	408512	13	NULL	NULL	0	NULL	thin-layer chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorbed lipid was extracted from the disks with ether and analyzed for wax esters by thin-layer chromatography .
	manualset3
155301	1	408513	13	NULL	NULL	0	NULL	absorption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorption , biotransformation and elimination of sulfinpyrazone , 1 , 2-diphenyl-3 , 5 - dioxo-4 - ( 2 ' - phenylsufinylethyl ) - pyrazolidine , have been studied by administration of single 200 mg oral doses of a 14C-labelled preparation to two male volunteers .
	manualset3
155302	2	408513	13	NULL	NULL	0	NULL	biotransformation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorption , biotransformation and elimination of sulfinpyrazone , 1 , 2-diphenyl-3 , 5 - dioxo-4 - ( 2 ' - phenylsufinylethyl ) - pyrazolidine , have been studied by administration of single 200 mg oral doses of a 14C-labelled preparation to two male volunteers .
	manualset3
155303	3	408513	13	NULL	NULL	0	NULL	elimination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorption , biotransformation and elimination of sulfinpyrazone , 1 , 2-diphenyl-3 , 5 - dioxo-4 - ( 2 ' - phenylsufinylethyl ) - pyrazolidine , have been studied by administration of single 200 mg oral doses of a 14C-labelled preparation to two male volunteers .
	manualset3
155304	4	408513	13	NULL	NULL	NULL	NULL	sulfinpyrazone	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The absorption , biotransformation and elimination of sulfinpyrazone , 1 , 2-diphenyl-3 , 5 - dioxo-4 - ( 2 ' - phenylsufinylethyl ) - pyrazolidine , have been studied by administration of single 200 mg oral doses of a 14C-labelled preparation to two male volunteers .
	manualset3
155305	5	408513	13	NULL	NULL	0	NULL	1 , 2-diphenyl-3 , 5 - dioxo-4 - ( 2 ' - phenylsufinylethyl ) - pyrazolidine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorption , biotransformation and elimination of sulfinpyrazone , 1 , 2-diphenyl-3 , 5 - dioxo-4 - ( 2 ' - phenylsufinylethyl ) - pyrazolidine , have been studied by administration of single 200 mg oral doses of a 14C-labelled preparation to two male volunteers .
	manualset3
155306	6	408513	13	NULL	NULL	0	NULL	administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorption , biotransformation and elimination of sulfinpyrazone , 1 , 2-diphenyl-3 , 5 - dioxo-4 - ( 2 ' - phenylsufinylethyl ) - pyrazolidine , have been studied by administration of single 200 mg oral doses of a 14C-labelled preparation to two male volunteers .
	manualset3
155307	7	408513	13	NULL	NULL	0	NULL	single 200 mg oral doses	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorption , biotransformation and elimination of sulfinpyrazone , 1 , 2-diphenyl-3 , 5 - dioxo-4 - ( 2 ' - phenylsufinylethyl ) - pyrazolidine , have been studied by administration of single 200 mg oral doses of a 14C-labelled preparation to two male volunteers .
	manualset3
155308	8	408513	13	NULL	NULL	0	NULL	14C-labelled preparation	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorption , biotransformation and elimination of sulfinpyrazone , 1 , 2-diphenyl-3 , 5 - dioxo-4 - ( 2 ' - phenylsufinylethyl ) - pyrazolidine , have been studied by administration of single 200 mg oral doses of a 14C-labelled preparation to two male volunteers .
	manualset3
155309	9	408513	13	NULL	NULL	0	NULL	two male volunteers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorption , biotransformation and elimination of sulfinpyrazone , 1 , 2-diphenyl-3 , 5 - dioxo-4 - ( 2 ' - phenylsufinylethyl ) - pyrazolidine , have been studied by administration of single 200 mg oral doses of a 14C-labelled preparation to two male volunteers .
	manualset3
155310	1	408514	13	NULL	NULL	0	NULL	absorption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorption , transport and distribution of alpha - ( 3H ) tocopherol were greatly decreased in protein deficiency .
	manualset3
155311	2	408514	13	NULL	NULL	0	NULL	transport	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorption , transport and distribution of alpha - ( 3H ) tocopherol were greatly decreased in protein deficiency .
	manualset3
155312	3	408514	13	NULL	NULL	0	NULL	distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorption , transport and distribution of alpha - ( 3H ) tocopherol were greatly decreased in protein deficiency .
	manualset3
155313	4	408514	13	NULL	NULL	0	NULL	alpha - ( 3H ) tocopherol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorption , transport and distribution of alpha - ( 3H ) tocopherol were greatly decreased in protein deficiency .
	manualset3
155314	5	408514	13	NULL	NULL	0	NULL	protein deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorption , transport and distribution of alpha - ( 3H ) tocopherol were greatly decreased in protein deficiency .
	manualset3
155315	1	408515	13	NULL	NULL	0	NULL	absorption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorption of a photon by the visual pigment-rhodopsin , a chromoprotein-causes a photo-chemical reaction , which is followed by a cascade of dark reactions of rhodopsin .
	manualset3
155316	2	408515	13	NULL	NULL	0	NULL	photon	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorption of a photon by the visual pigment-rhodopsin , a chromoprotein-causes a photo-chemical reaction , which is followed by a cascade of dark reactions of rhodopsin .
	manualset3
155317	3	408515	13	NULL	NULL	0	NULL	visual pigment-rhodopsin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorption of a photon by the visual pigment-rhodopsin , a chromoprotein-causes a photo-chemical reaction , which is followed by a cascade of dark reactions of rhodopsin .
	manualset3
155318	4	408515	13	NULL	NULL	0	NULL	photo-chemical reaction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorption of a photon by the visual pigment-rhodopsin , a chromoprotein-causes a photo-chemical reaction , which is followed by a cascade of dark reactions of rhodopsin .
	manualset3
155319	5	408515	13	NULL	NULL	0	NULL	cascade of dark reactions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorption of a photon by the visual pigment-rhodopsin , a chromoprotein-causes a photo-chemical reaction , which is followed by a cascade of dark reactions of rhodopsin .
	manualset3
155320	6	408515	13	NULL	NULL	0	NULL	rhodopsin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorption of a photon by the visual pigment-rhodopsin , a chromoprotein-causes a photo-chemical reaction , which is followed by a cascade of dark reactions of rhodopsin .
	manualset3
155321	1	408516	13	NULL	NULL	0	NULL	absorption 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorption of atovaquone from tablets was examined in 12 healthy male volunteers after an overnight fast , following toast alone , toast with 28 g butter ( LOFAT ) , or toast with 56 g butter ( HIFAT ) .
	manualset3
155322	2	408516	13	NULL	NULL	0	NULL	atovaquone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorption of atovaquone from tablets was examined in 12 healthy male volunteers after an overnight fast , following toast alone , toast with 28 g butter ( LOFAT ) , or toast with 56 g butter ( HIFAT ) .
	manualset3
155323	3	408516	13	NULL	NULL	0	NULL	tablets	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorption of atovaquone from tablets was examined in 12 healthy male volunteers after an overnight fast , following toast alone , toast with 28 g butter ( LOFAT ) , or toast with 56 g butter ( HIFAT ) .
	manualset3
155324	4	408516	13	NULL	NULL	0	NULL	12 healthy male volunteers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorption of atovaquone from tablets was examined in 12 healthy male volunteers after an overnight fast , following toast alone , toast with 28 g butter ( LOFAT ) , or toast with 56 g butter ( HIFAT ) .
	manualset3
155325	5	408516	13	NULL	NULL	0	NULL	toast	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorption of atovaquone from tablets was examined in 12 healthy male volunteers after an overnight fast , following toast alone , toast with 28 g butter ( LOFAT ) , or toast with 56 g butter ( HIFAT ) .
	manualset3
155326	6	408516	13	NULL	NULL	0	NULL	toast	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorption of atovaquone from tablets was examined in 12 healthy male volunteers after an overnight fast , following toast alone , toast with 28 g butter ( LOFAT ) , or toast with 56 g butter ( HIFAT ) .
	manualset3
155327	7	408516	13	NULL	NULL	0	NULL	28 g butter 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorption of atovaquone from tablets was examined in 12 healthy male volunteers after an overnight fast , following toast alone , toast with 28 g butter ( LOFAT ) , or toast with 56 g butter ( HIFAT ) .
	manualset3
155328	8	408516	13	NULL	NULL	0	NULL	LOFAT	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorption of atovaquone from tablets was examined in 12 healthy male volunteers after an overnight fast , following toast alone , toast with 28 g butter ( LOFAT ) , or toast with 56 g butter ( HIFAT ) .
	manualset3
155329	9	408516	13	NULL	NULL	0	NULL	toast	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorption of atovaquone from tablets was examined in 12 healthy male volunteers after an overnight fast , following toast alone , toast with 28 g butter ( LOFAT ) , or toast with 56 g butter ( HIFAT ) .
	manualset3
155330	10	408516	13	NULL	NULL	0	NULL	56 g butter 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorption of atovaquone from tablets was examined in 12 healthy male volunteers after an overnight fast , following toast alone , toast with 28 g butter ( LOFAT ) , or toast with 56 g butter ( HIFAT ) .
	manualset3
155331	11	408516	13	NULL	NULL	0	NULL	HIFAT	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The absorption of atovaquone from tablets was examined in 12 healthy male volunteers after an overnight fast , following toast alone , toast with 28 g butter ( LOFAT ) , or toast with 56 g butter ( HIFAT ) .
	manualset3
155332	1	408517	13	NULL	NULL	0	NULL	abundance 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The abundance of ribosomal proteins paralleled total protein content during refeeding in both control and rapamycin-injected rats .
	manualset3
155333	2	408517	13	NULL	NULL	0	NULL	ribosomal proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The abundance of ribosomal proteins paralleled total protein content during refeeding in both control and rapamycin-injected rats .
	manualset3
155334	3	408517	13	NULL	NULL	0	NULL	total protein content 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The abundance of ribosomal proteins paralleled total protein content during refeeding in both control and rapamycin-injected rats .
	manualset3
155335	4	408517	13	NULL	NULL	0	NULL	control rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The abundance of ribosomal proteins paralleled total protein content during refeeding in both control and rapamycin-injected rats .
	manualset3
155336	5	408517	13	NULL	NULL	0	NULL	rapamycin-injected rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The abundance of ribosomal proteins paralleled total protein content during refeeding in both control and rapamycin-injected rats .
	manualset3
155337	1	408518	13	NULL	NULL	0	NULL	abundance	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The abundance of the genera Achaeta and Enchytraeus was not affected .
	manualset3
155338	2	408518	13	NULL	NULL	0	NULL	genera Achaeta 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The abundance of the genera Achaeta and Enchytraeus was not affected .
	manualset3
155339	3	408518	13	NULL	NULL	0	NULL	Enchytraeus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The abundance of the genera Achaeta and Enchytraeus was not affected .
	manualset3
155340	1	408519	13	NULL	NULL	0	NULL	abuse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The abuse of the designer amphetamines such as 3 , 4-methylenedioxymethamphetamine ( MDMA ) is increasing throughout the world .
	manualset3
155341	2	408519	13	NULL	NULL	0	NULL	designer amphetamines 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The abuse of the designer amphetamines such as 3 , 4-methylenedioxymethamphetamine ( MDMA ) is increasing throughout the world .
	manualset3
155342	3	408519	13	NULL	NULL	0	NULL	3 , 4-methylenedioxymethamphetamine ( MDMA ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The abuse of the designer amphetamines such as 3 , 4-methylenedioxymethamphetamine ( MDMA ) is increasing throughout the world .
	manualset3
155343	4	408519	13	NULL	NULL	0	NULL	world 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The abuse of the designer amphetamines such as 3 , 4-methylenedioxymethamphetamine ( MDMA ) is increasing throughout the world .
	manualset3
155344	1	408520	13	NULL	NULL	0	NULL	accent 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The accent is placed on its most significant aspects , such as : difficulties of differential diagnosis with other repletion defect imagen in the excretory tract and their frequent association to other diseases .
	manualset3
155345	2	408520	13	NULL	NULL	0	NULL	aspects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The accent is placed on its most significant aspects , such as : difficulties of differential diagnosis with other repletion defect imagen in the excretory tract and their frequent association to other diseases .
	manualset3
155346	3	408520	13	NULL	NULL	0	NULL	difficulties	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The accent is placed on its most significant aspects , such as : difficulties of differential diagnosis with other repletion defect imagen in the excretory tract and their frequent association to other diseases .
	manualset3
155347	4	408520	13	NULL	NULL	0	NULL	differential diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The accent is placed on its most significant aspects , such as : difficulties of differential diagnosis with other repletion defect imagen in the excretory tract and their frequent association to other diseases .
	manualset3
155348	5	408520	13	NULL	NULL	0	NULL	repletion defect imagen	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The accent is placed on its most significant aspects , such as : difficulties of differential diagnosis with other repletion defect imagen in the excretory tract and their frequent association to other diseases .
	manualset3
155349	6	408520	13	NULL	NULL	0	NULL	excretory tract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The accent is placed on its most significant aspects , such as : difficulties of differential diagnosis with other repletion defect imagen in the excretory tract and their frequent association to other diseases .
	manualset3
155350	7	408520	13	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The accent is placed on its most significant aspects , such as : difficulties of differential diagnosis with other repletion defect imagen in the excretory tract and their frequent association to other diseases .
	manualset3
155351	8	408520	13	NULL	NULL	0	NULL	diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The accent is placed on its most significant aspects , such as : difficulties of differential diagnosis with other repletion defect imagen in the excretory tract and their frequent association to other diseases .
	manualset3
155352	1	408521	13	NULL	NULL	0	NULL	accomplishment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The accomplishment of air-stability was attributed to the combined effect of the low-lying LUMO energy level and the molecular arrangements in the solid state , avoiding both the quenching of electron carriers and the intrusion of oxygen and/or moisture .
	manualset3
155353	2	408521	13	NULL	NULL	0	NULL	air-stability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The accomplishment of air-stability was attributed to the combined effect of the low-lying LUMO energy level and the molecular arrangements in the solid state , avoiding both the quenching of electron carriers and the intrusion of oxygen and/or moisture .
	manualset3
155354	3	408521	13	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The accomplishment of air-stability was attributed to the combined effect of the low-lying LUMO energy level and the molecular arrangements in the solid state , avoiding both the quenching of electron carriers and the intrusion of oxygen and/or moisture .
	manualset3
155355	4	408521	13	NULL	NULL	0	NULL	 low-lying LUMO energy level	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The accomplishment of air-stability was attributed to the combined effect of the low-lying LUMO energy level and the molecular arrangements in the solid state , avoiding both the quenching of electron carriers and the intrusion of oxygen and/or moisture .
	manualset3
155356	5	408521	13	NULL	NULL	0	NULL	molecular arrangements	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The accomplishment of air-stability was attributed to the combined effect of the low-lying LUMO energy level and the molecular arrangements in the solid state , avoiding both the quenching of electron carriers and the intrusion of oxygen and/or moisture .
	manualset3
155357	6	408521	13	NULL	NULL	0	NULL	solid state	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The accomplishment of air-stability was attributed to the combined effect of the low-lying LUMO energy level and the molecular arrangements in the solid state , avoiding both the quenching of electron carriers and the intrusion of oxygen and/or moisture .
	manualset3
155358	7	408521	13	NULL	NULL	0	NULL	quenching	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The accomplishment of air-stability was attributed to the combined effect of the low-lying LUMO energy level and the molecular arrangements in the solid state , avoiding both the quenching of electron carriers and the intrusion of oxygen and/or moisture .
	manualset3
155359	8	408521	13	NULL	NULL	NULL	NULL	electron carriers	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The accomplishment of air-stability was attributed to the combined effect of the low-lying LUMO energy level and the molecular arrangements in the solid state , avoiding both the quenching of electron carriers and the intrusion of oxygen and/or moisture .
	manualset3
155360	9	408521	13	NULL	NULL	0	NULL	intrusion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The accomplishment of air-stability was attributed to the combined effect of the low-lying LUMO energy level and the molecular arrangements in the solid state , avoiding both the quenching of electron carriers and the intrusion of oxygen and/or moisture .
	manualset3
155361	10	408521	13	NULL	NULL	0	NULL	oxygen	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The accomplishment of air-stability was attributed to the combined effect of the low-lying LUMO energy level and the molecular arrangements in the solid state , avoiding both the quenching of electron carriers and the intrusion of oxygen and/or moisture .
	manualset3
155362	11	408521	13	NULL	NULL	0	NULL	moisture 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The accomplishment of air-stability was attributed to the combined effect of the low-lying LUMO energy level and the molecular arrangements in the solid state , avoiding both the quenching of electron carriers and the intrusion of oxygen and/or moisture .
	manualset3
155363	1	408522	13	NULL	NULL	0	NULL	accuracy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The accuracy and cost savings of pooling specimens prior to testing for Chlamydia trachomatis by PCR were evaluated with genital and urine specimens ( n = 2 , 600 ) .
	manualset3
155364	2	408522	13	NULL	NULL	0	NULL	cost savings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The accuracy and cost savings of pooling specimens prior to testing for Chlamydia trachomatis by PCR were evaluated with genital and urine specimens ( n = 2 , 600 ) .
	manualset3
155365	3	408522	13	NULL	NULL	0	NULL	 specimens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The accuracy and cost savings of pooling specimens prior to testing for Chlamydia trachomatis by PCR were evaluated with genital and urine specimens ( n = 2 , 600 ) .
	manualset3
155366	4	408522	13	NULL	NULL	0	NULL	testing 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The accuracy and cost savings of pooling specimens prior to testing for Chlamydia trachomatis by PCR were evaluated with genital and urine specimens ( n = 2 , 600 ) .
	manualset3
155367	5	408522	13	NULL	NULL	0	NULL	Chlamydia trachomatis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The accuracy and cost savings of pooling specimens prior to testing for Chlamydia trachomatis by PCR were evaluated with genital and urine specimens ( n = 2 , 600 ) .
	manualset3
155368	6	408522	13	NULL	NULL	0	NULL	PCR 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The accuracy and cost savings of pooling specimens prior to testing for Chlamydia trachomatis by PCR were evaluated with genital and urine specimens ( n = 2 , 600 ) .
	manualset3
155369	7	408522	13	NULL	NULL	0	NULL	genital specimens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The accuracy and cost savings of pooling specimens prior to testing for Chlamydia trachomatis by PCR were evaluated with genital and urine specimens ( n = 2 , 600 ) .
	manualset3
155370	8	408522	13	NULL	NULL	0	NULL	urine specimens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The accuracy and cost savings of pooling specimens prior to testing for Chlamydia trachomatis by PCR were evaluated with genital and urine specimens ( n = 2 , 600 ) .
	manualset3
155371	9	408522	13	NULL	NULL	0	NULL	n = 2 , 600	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The accuracy and cost savings of pooling specimens prior to testing for Chlamydia trachomatis by PCR were evaluated with genital and urine specimens ( n = 2 , 600 ) .
	manualset3
155372	1	408523	13	NULL	NULL	0	NULL	accuracy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The accuracy of auto-CAD was compared with the formal radiology report .
	manualset3
155373	2	408523	13	NULL	NULL	0	NULL	auto-CAD	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The accuracy of auto-CAD was compared with the formal radiology report .
	manualset3
155374	3	408523	13	NULL	NULL	0	NULL	radiology report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The accuracy of auto-CAD was compared with the formal radiology report .
	manualset3
155412	1	408524	13	NULL	NULL	0	NULL	acetic-acid-induced vascular permeability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The acetic-acid-induced vascular permeability , erythrocyte membrane stabilization , release of proinflammatory mediators ( nitric oxide and prostaglandin E ( 2 ) ) , and cytokines ( tumor necrosis factor - , and interleukins-1 and -6 ) from lipopolysaccharide-stimulated human monocytic cell lines were assessed to understand the mechanism of action .
	manualset3
155413	2	408524	13	NULL	NULL	0	NULL	erythrocyte membrane stabilization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The acetic-acid-induced vascular permeability , erythrocyte membrane stabilization , release of proinflammatory mediators ( nitric oxide and prostaglandin E ( 2 ) ) , and cytokines ( tumor necrosis factor - , and interleukins-1 and -6 ) from lipopolysaccharide-stimulated human monocytic cell lines were assessed to understand the mechanism of action .
	manualset3
155415	3	408524	13	NULL	NULL	0	NULL	release of proinflammatory mediators 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The acetic-acid-induced vascular permeability , erythrocyte membrane stabilization , release of proinflammatory mediators ( nitric oxide and prostaglandin E ( 2 ) ) , and cytokines ( tumor necrosis factor - , and interleukins-1 and -6 ) from lipopolysaccharide-stimulated human monocytic cell lines were assessed to understand the mechanism of action .
	manualset3
155416	4	408524	13	NULL	NULL	0	NULL	nitric oxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The acetic-acid-induced vascular permeability , erythrocyte membrane stabilization , release of proinflammatory mediators ( nitric oxide and prostaglandin E ( 2 ) ) , and cytokines ( tumor necrosis factor - , and interleukins-1 and -6 ) from lipopolysaccharide-stimulated human monocytic cell lines were assessed to understand the mechanism of action .
	manualset3
155421	5	408524	13	NULL	NULL	0	NULL	prostaglandin E ( 2 ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The acetic-acid-induced vascular permeability , erythrocyte membrane stabilization , release of proinflammatory mediators ( nitric oxide and prostaglandin E ( 2 ) ) , and cytokines ( tumor necrosis factor - , and interleukins-1 and -6 ) from lipopolysaccharide-stimulated human monocytic cell lines were assessed to understand the mechanism of action .
	manualset3
155423	6	408524	13	NULL	NULL	0	NULL	cytokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The acetic-acid-induced vascular permeability , erythrocyte membrane stabilization , release of proinflammatory mediators ( nitric oxide and prostaglandin E ( 2 ) ) , and cytokines ( tumor necrosis factor - , and interleukins-1 and -6 ) from lipopolysaccharide-stimulated human monocytic cell lines were assessed to understand the mechanism of action .
	manualset3
155424	7	408524	13	NULL	NULL	0	NULL	tumor necrosis factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The acetic-acid-induced vascular permeability , erythrocyte membrane stabilization , release of proinflammatory mediators ( nitric oxide and prostaglandin E ( 2 ) ) , and cytokines ( tumor necrosis factor - , and interleukins-1 and -6 ) from lipopolysaccharide-stimulated human monocytic cell lines were assessed to understand the mechanism of action .
	manualset3
155425	8	408524	13	NULL	NULL	0	NULL	 interleukins-1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The acetic-acid-induced vascular permeability , erythrocyte membrane stabilization , release of proinflammatory mediators ( nitric oxide and prostaglandin E ( 2 ) ) , and cytokines ( tumor necrosis factor - , and interleukins-1 and -6 ) from lipopolysaccharide-stimulated human monocytic cell lines were assessed to understand the mechanism of action .
	manualset3
155426	9	408524	13	NULL	NULL	0	NULL	 interleukins-6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The acetic-acid-induced vascular permeability , erythrocyte membrane stabilization , release of proinflammatory mediators ( nitric oxide and prostaglandin E ( 2 ) ) , and cytokines ( tumor necrosis factor - , and interleukins-1 and -6 ) from lipopolysaccharide-stimulated human monocytic cell lines were assessed to understand the mechanism of action .
	manualset3
155428	10	408524	13	NULL	NULL	0	NULL	human monocytic cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The acetic-acid-induced vascular permeability , erythrocyte membrane stabilization , release of proinflammatory mediators ( nitric oxide and prostaglandin E ( 2 ) ) , and cytokines ( tumor necrosis factor - , and interleukins-1 and -6 ) from lipopolysaccharide-stimulated human monocytic cell lines were assessed to understand the mechanism of action .
	manualset3
155429	11	408524	13	NULL	NULL	0	NULL	mechanism of action 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The acetic-acid-induced vascular permeability , erythrocyte membrane stabilization , release of proinflammatory mediators ( nitric oxide and prostaglandin E ( 2 ) ) , and cytokines ( tumor necrosis factor - , and interleukins-1 and -6 ) from lipopolysaccharide-stimulated human monocytic cell lines were assessed to understand the mechanism of action .
	manualset3
155430	1	408525	13	NULL	NULL	0	NULL	impedance characteristics	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The achieved impedance characteristics depend on the conditions during the learning process .
	manualset3
155431	2	408525	13	NULL	NULL	0	NULL	conditions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The achieved impedance characteristics depend on the conditions during the learning process .
	manualset3
155432	3	408525	13	NULL	NULL	0	NULL	learning process	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The achieved impedance characteristics depend on the conditions during the learning process .
	manualset3
155433	1	408526	13	NULL	NULL	0	NULL	reporter construct 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A reporter construct consisting of 13 kilobases of the human CYP3A4 promoter controlling the firefly luciferase gene was used to generate a transgenic mouse line ( FVB/N-Tg ( CYP3A4-luc ) Xen ) .
	manualset3
155434	2	408526	13	NULL	NULL	0	NULL	13 kilobases	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A reporter construct consisting of 13 kilobases of the human CYP3A4 promoter controlling the firefly luciferase gene was used to generate a transgenic mouse line ( FVB/N-Tg ( CYP3A4-luc ) Xen ) .
	manualset3
155435	3	408526	13	NULL	NULL	0	NULL	 human CYP3A4 promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A reporter construct consisting of 13 kilobases of the human CYP3A4 promoter controlling the firefly luciferase gene was used to generate a transgenic mouse line ( FVB/N-Tg ( CYP3A4-luc ) Xen ) .
	manualset3
155436	4	408526	13	NULL	NULL	0	NULL	firefly luciferase gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A reporter construct consisting of 13 kilobases of the human CYP3A4 promoter controlling the firefly luciferase gene was used to generate a transgenic mouse line ( FVB/N-Tg ( CYP3A4-luc ) Xen ) .
	manualset3
155437	5	408526	13	NULL	NULL	0	NULL	transgenic mouse line 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A reporter construct consisting of 13 kilobases of the human CYP3A4 promoter controlling the firefly luciferase gene was used to generate a transgenic mouse line ( FVB/N-Tg ( CYP3A4-luc ) Xen ) .
	manualset3
155438	6	408526	13	NULL	NULL	0	NULL	( FVB/N-Tg ( CYP3A4-luc ) Xen )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A reporter construct consisting of 13 kilobases of the human CYP3A4 promoter controlling the firefly luciferase gene was used to generate a transgenic mouse line ( FVB/N-Tg ( CYP3A4-luc ) Xen ) .
	manualset3
155439	1	408527	13	NULL	NULL	0	NULL	acidurance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The acidurance of glycolysis by intact cells of Streptococcus mutans GS-5 , Streptococcus salivarius ATCC 25925 , and Streptococcus sanguis NCTC 10904 was found to be highly dependent on membrane functions affected by gramicidin , which increases the proton permeability of cell membranes .
	manualset3
155440	2	408527	13	NULL	NULL	0	NULL	glycolysis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The acidurance of glycolysis by intact cells of Streptococcus mutans GS-5 , Streptococcus salivarius ATCC 25925 , and Streptococcus sanguis NCTC 10904 was found to be highly dependent on membrane functions affected by gramicidin , which increases the proton permeability of cell membranes .
	manualset3
155441	3	408527	13	NULL	NULL	0	NULL	intact cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The acidurance of glycolysis by intact cells of Streptococcus mutans GS-5 , Streptococcus salivarius ATCC 25925 , and Streptococcus sanguis NCTC 10904 was found to be highly dependent on membrane functions affected by gramicidin , which increases the proton permeability of cell membranes .
	manualset3
155442	4	408527	13	NULL	NULL	0	NULL	Streptococcus mutans GS-5	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The acidurance of glycolysis by intact cells of Streptococcus mutans GS-5 , Streptococcus salivarius ATCC 25925 , and Streptococcus sanguis NCTC 10904 was found to be highly dependent on membrane functions affected by gramicidin , which increases the proton permeability of cell membranes .
	manualset3
155443	5	408527	13	NULL	NULL	0	NULL	Streptococcus salivarius ATCC 25925	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The acidurance of glycolysis by intact cells of Streptococcus mutans GS-5 , Streptococcus salivarius ATCC 25925 , and Streptococcus sanguis NCTC 10904 was found to be highly dependent on membrane functions affected by gramicidin , which increases the proton permeability of cell membranes .
	manualset3
155444	6	408527	13	NULL	NULL	0	NULL	Streptococcus sanguis NCTC 10904	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The acidurance of glycolysis by intact cells of Streptococcus mutans GS-5 , Streptococcus salivarius ATCC 25925 , and Streptococcus sanguis NCTC 10904 was found to be highly dependent on membrane functions affected by gramicidin , which increases the proton permeability of cell membranes .
	manualset3
155445	7	408527	13	NULL	NULL	0	NULL	membrane functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The acidurance of glycolysis by intact cells of Streptococcus mutans GS-5 , Streptococcus salivarius ATCC 25925 , and Streptococcus sanguis NCTC 10904 was found to be highly dependent on membrane functions affected by gramicidin , which increases the proton permeability of cell membranes .
	manualset3
155446	8	408527	13	NULL	NULL	0	NULL	gramicidin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The acidurance of glycolysis by intact cells of Streptococcus mutans GS-5 , Streptococcus salivarius ATCC 25925 , and Streptococcus sanguis NCTC 10904 was found to be highly dependent on membrane functions affected by gramicidin , which increases the proton permeability of cell membranes .
	manualset3
155447	9	408527	13	NULL	NULL	0	NULL	proton permeability 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The acidurance of glycolysis by intact cells of Streptococcus mutans GS-5 , Streptococcus salivarius ATCC 25925 , and Streptococcus sanguis NCTC 10904 was found to be highly dependent on membrane functions affected by gramicidin , which increases the proton permeability of cell membranes .
	manualset3
155449	10	408527	13	NULL	NULL	0	NULL	cell membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The acidurance of glycolysis by intact cells of Streptococcus mutans GS-5 , Streptococcus salivarius ATCC 25925 , and Streptococcus sanguis NCTC 10904 was found to be highly dependent on membrane functions affected by gramicidin , which increases the proton permeability of cell membranes .
	manualset3
155452	1	408528	13	NULL	NULL	0	NULL	condition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The acquired condition is mainly due to alloimmunization against HLA-antigen on leucocytes in the transfused platelets or to non-immunological factors , e.g. fever , infections , bleedings , antibodies or splenomegaly .
	manualset3
155454	2	408528	13	NULL	NULL	0	NULL	HLA-antigen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The acquired condition is mainly due to alloimmunization against HLA-antigen on leucocytes in the transfused platelets or to non-immunological factors , e.g. fever , infections , bleedings , antibodies or splenomegaly .
	manualset3
155455	3	408528	13	NULL	NULL	0	NULL	leucocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The acquired condition is mainly due to alloimmunization against HLA-antigen on leucocytes in the transfused platelets or to non-immunological factors , e.g. fever , infections , bleedings , antibodies or splenomegaly .
	manualset3
155456	4	408528	13	NULL	NULL	0	NULL	platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The acquired condition is mainly due to alloimmunization against HLA-antigen on leucocytes in the transfused platelets or to non-immunological factors , e.g. fever , infections , bleedings , antibodies or splenomegaly .
	manualset3
155457	5	408528	13	NULL	NULL	0	NULL	non-immunological factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The acquired condition is mainly due to alloimmunization against HLA-antigen on leucocytes in the transfused platelets or to non-immunological factors , e.g. fever , infections , bleedings , antibodies or splenomegaly .
	manualset3
155458	6	408528	13	NULL	NULL	0	NULL	fever	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The acquired condition is mainly due to alloimmunization against HLA-antigen on leucocytes in the transfused platelets or to non-immunological factors , e.g. fever , infections , bleedings , antibodies or splenomegaly .
	manualset3
155459	7	408528	13	NULL	NULL	0	NULL	infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The acquired condition is mainly due to alloimmunization against HLA-antigen on leucocytes in the transfused platelets or to non-immunological factors , e.g. fever , infections , bleedings , antibodies or splenomegaly .
	manualset3
155460	8	408528	13	NULL	NULL	0	NULL	bleedings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The acquired condition is mainly due to alloimmunization against HLA-antigen on leucocytes in the transfused platelets or to non-immunological factors , e.g. fever , infections , bleedings , antibodies or splenomegaly .
	manualset3
155461	9	408528	13	NULL	NULL	0	NULL	antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The acquired condition is mainly due to alloimmunization against HLA-antigen on leucocytes in the transfused platelets or to non-immunological factors , e.g. fever , infections , bleedings , antibodies or splenomegaly .
	manualset3
155462	10	408528	13	NULL	NULL	0	NULL	splenomegaly	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The acquired condition is mainly due to alloimmunization against HLA-antigen on leucocytes in the transfused platelets or to non-immunological factors , e.g. fever , infections , bleedings , antibodies or splenomegaly .
	manualset3
155469	1	408529	13	NULL	NULL	0	NULL	acronym ICER 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The acronym ICER ( inducible cAMP early repressor ) refers to a group of four proteins produced from the CREM/ICER gene due to use of an internal promoter ( P2 ) placed in an intron of the CREM ( cAMP responsive element modulator ) gene .
	manualset3
155470	2	408529	13	NULL	NULL	0	NULL	inducible cAMP early repressor 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The acronym ICER ( inducible cAMP early repressor ) refers to a group of four proteins produced from the CREM/ICER gene due to use of an internal promoter ( P2 ) placed in an intron of the CREM ( cAMP responsive element modulator ) gene .
	manualset3
155471	3	408529	13	NULL	NULL	0	NULL	 group of four proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The acronym ICER ( inducible cAMP early repressor ) refers to a group of four proteins produced from the CREM/ICER gene due to use of an internal promoter ( P2 ) placed in an intron of the CREM ( cAMP responsive element modulator ) gene .
	manualset3
155472	4	408529	13	NULL	NULL	0	NULL	CREM/ICER gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The acronym ICER ( inducible cAMP early repressor ) refers to a group of four proteins produced from the CREM/ICER gene due to use of an internal promoter ( P2 ) placed in an intron of the CREM ( cAMP responsive element modulator ) gene .
	manualset3
155473	5	408529	13	NULL	NULL	0	NULL	use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The acronym ICER ( inducible cAMP early repressor ) refers to a group of four proteins produced from the CREM/ICER gene due to use of an internal promoter ( P2 ) placed in an intron of the CREM ( cAMP responsive element modulator ) gene .
	manualset3
155474	6	408529	13	NULL	NULL	0	NULL	 internal promoter ( P2 ) 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The acronym ICER ( inducible cAMP early repressor ) refers to a group of four proteins produced from the CREM/ICER gene due to use of an internal promoter ( P2 ) placed in an intron of the CREM ( cAMP responsive element modulator ) gene .
	manualset3
155475	7	408529	13	NULL	NULL	0	NULL	intron	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The acronym ICER ( inducible cAMP early repressor ) refers to a group of four proteins produced from the CREM/ICER gene due to use of an internal promoter ( P2 ) placed in an intron of the CREM ( cAMP responsive element modulator ) gene .
	manualset3
155477	8	408529	13	NULL	NULL	0	NULL	CREM ( cAMP responsive element modulator ) gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The acronym ICER ( inducible cAMP early repressor ) refers to a group of four proteins produced from the CREM/ICER gene due to use of an internal promoter ( P2 ) placed in an intron of the CREM ( cAMP responsive element modulator ) gene .
	manualset3
155479	1	408530	13	NULL	NULL	0	NULL	action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of TGF-beta2 could be abolished by cycloheximide or EGTA , suggesting the requirement of a newly synthesized protein and extracellular Ca2 + .
	manualset3
155480	2	408530	13	NULL	NULL	0	NULL	TGF-beta2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of TGF-beta2 could be abolished by cycloheximide or EGTA , suggesting the requirement of a newly synthesized protein and extracellular Ca2 + .
	manualset3
155482	3	408530	13	NULL	NULL	0	NULL	cycloheximide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of TGF-beta2 could be abolished by cycloheximide or EGTA , suggesting the requirement of a newly synthesized protein and extracellular Ca2 + .
	manualset3
155483	4	408530	13	NULL	NULL	0	NULL	EGTA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of TGF-beta2 could be abolished by cycloheximide or EGTA , suggesting the requirement of a newly synthesized protein and extracellular Ca2 + .
	manualset3
155484	5	408530	13	NULL	NULL	0	NULL	requirement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of TGF-beta2 could be abolished by cycloheximide or EGTA , suggesting the requirement of a newly synthesized protein and extracellular Ca2 + .
	manualset3
155486	6	408530	13	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of TGF-beta2 could be abolished by cycloheximide or EGTA , suggesting the requirement of a newly synthesized protein and extracellular Ca2 + .
	manualset3
155487	7	408530	13	NULL	NULL	0	NULL	extracellular Ca2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of TGF-beta2 could be abolished by cycloheximide or EGTA , suggesting the requirement of a newly synthesized protein and extracellular Ca2 + .
	manualset3
140090	1	408531	5	NULL	NULL	0	NULL	US 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of US converts CL at very low temperatures ( 70-110 degrees C ) and water content , in comparison with silent conditions where CL was unconverted .
	manualset3
140091	2	408531	5	NULL	NULL	0	NULL	CL 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of US converts CL at very low temperatures ( 70-110 degrees C ) and water content , in comparison with silent conditions where CL was unconverted .
	manualset3
140092	3	408531	5	NULL	NULL	0	NULL	low temperatures 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of US converts CL at very low temperatures ( 70-110 degrees C ) and water content , in comparison with silent conditions where CL was unconverted .
	manualset3
140093	4	408531	5	NULL	NULL	0	NULL	70-110 degrees C 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of US converts CL at very low temperatures ( 70-110 degrees C ) and water content , in comparison with silent conditions where CL was unconverted .
	manualset3
140094	5	408531	5	NULL	NULL	0	NULL	water content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of US converts CL at very low temperatures ( 70-110 degrees C ) and water content , in comparison with silent conditions where CL was unconverted .
	manualset3
140095	6	408531	5	NULL	NULL	0	NULL	comparison 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of US converts CL at very low temperatures ( 70-110 degrees C ) and water content , in comparison with silent conditions where CL was unconverted .
	manualset3
140096	7	408531	5	NULL	NULL	0	NULL	silent conditions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of US converts CL at very low temperatures ( 70-110 degrees C ) and water content , in comparison with silent conditions where CL was unconverted .
	manualset3
140097	8	408531	5	NULL	NULL	0	NULL	CL	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of US converts CL at very low temperatures ( 70-110 degrees C ) and water content , in comparison with silent conditions where CL was unconverted .
	manualset3
142891	9	408531	5	NULL	NULL	0	NULL	action 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of US converts CL at very low temperatures ( 70-110 degrees C ) and water content , in comparison with silent conditions where CL was unconverted .
	manualset3
140098	1	408532	5	NULL	NULL	0	NULL	action 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of agents inhibiting evoked transmitter release was investigated by analyzing the Ca2 + secretion relationship , electrophysiologically and biochemically , and by measuring the stimulation-induced 45Ca accumulation in the tissue .
	manualset3
140099	2	408532	5	NULL	NULL	0	NULL	agents 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of agents inhibiting evoked transmitter release was investigated by analyzing the Ca2 + secretion relationship , electrophysiologically and biochemically , and by measuring the stimulation-induced 45Ca accumulation in the tissue .
	manualset3
140100	3	408532	5	NULL	NULL	0	NULL	transmitter release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of agents inhibiting evoked transmitter release was investigated by analyzing the Ca2 + secretion relationship , electrophysiologically and biochemically , and by measuring the stimulation-induced 45Ca accumulation in the tissue .
	manualset3
140101	4	408532	5	NULL	NULL	0	NULL	 Ca2 + secretion relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of agents inhibiting evoked transmitter release was investigated by analyzing the Ca2 + secretion relationship , electrophysiologically and biochemically , and by measuring the stimulation-induced 45Ca accumulation in the tissue .
	manualset3
140102	5	408532	5	NULL	NULL	0	NULL	stimulation-induced 45Ca accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of agents inhibiting evoked transmitter release was investigated by analyzing the Ca2 + secretion relationship , electrophysiologically and biochemically , and by measuring the stimulation-induced 45Ca accumulation in the tissue .
	manualset3
140103	6	408532	5	NULL	NULL	0	NULL	tissue 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of agents inhibiting evoked transmitter release was investigated by analyzing the Ca2 + secretion relationship , electrophysiologically and biochemically , and by measuring the stimulation-induced 45Ca accumulation in the tissue .
	manualset3
140104	1	408533	5	NULL	NULL	0	NULL	action 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of androgens in regulating development and growth is mediated by androgen receptor ( AR ) .
	manualset3
140105	2	408533	5	NULL	NULL	0	NULL	androgens 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of androgens in regulating development and growth is mediated by androgen receptor ( AR ) .
	manualset3
140106	3	408533	5	NULL	NULL	0	NULL	development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of androgens in regulating development and growth is mediated by androgen receptor ( AR ) .
	manualset3
140107	4	408533	5	NULL	NULL	0	NULL	growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of androgens in regulating development and growth is mediated by androgen receptor ( AR ) .
	manualset3
140108	5	408533	5	NULL	NULL	0	NULL	androgen receptor ( AR )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of androgens in regulating development and growth is mediated by androgen receptor ( AR ) .
	manualset3
140109	1	408534	5	NULL	NULL	0	NULL	action 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of insulin was attenuated by removal of calcium chloride from the bathing medium .
	manualset3
140110	2	408534	5	NULL	NULL	0	NULL	insulin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of insulin was attenuated by removal of calcium chloride from the bathing medium .
	manualset3
140111	3	408534	5	NULL	NULL	0	NULL	calcium chloride 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of insulin was attenuated by removal of calcium chloride from the bathing medium .
	manualset3
140112	4	408534	5	NULL	NULL	0	NULL	bathing medium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of insulin was attenuated by removal of calcium chloride from the bathing medium .
	manualset3
140113	1	408535	5	NULL	NULL	0	NULL	action 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of phospholipase C on muscle microsomes : a correlation of electron microscope and biochemical data .
	manualset3
140114	2	408535	5	NULL	NULL	0	NULL	phospholipase C 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of phospholipase C on muscle microsomes : a correlation of electron microscope and biochemical data .
	manualset3
140115	3	408535	5	NULL	NULL	0	NULL	muscle microsomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of phospholipase C on muscle microsomes : a correlation of electron microscope and biochemical data .
	manualset3
140116	4	408535	5	NULL	NULL	0	NULL	correlation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of phospholipase C on muscle microsomes : a correlation of electron microscope and biochemical data .
	manualset3
140117	5	408535	5	NULL	NULL	0	NULL	electron microscope	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of phospholipase C on muscle microsomes : a correlation of electron microscope and biochemical data .
	manualset3
140118	6	408535	5	NULL	NULL	0	NULL	biochemical data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of phospholipase C on muscle microsomes : a correlation of electron microscope and biochemical data .
	manualset3
140119	1	408536	5	NULL	NULL	0	NULL	action 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of protovertarines A and B , which stimulate carotid sinus baroreceptors and vagal sensory endings in the heart as well as pulmonary bed , were assessed on spontaneous and postsigh central sleep apneas in freely moving Sprague-Dawley rats .
	manualset3
140120	2	408536	5	NULL	NULL	0	NULL	protovertarine A	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of protovertarines A and B , which stimulate carotid sinus baroreceptors and vagal sensory endings in the heart as well as pulmonary bed , were assessed on spontaneous and postsigh central sleep apneas in freely moving Sprague-Dawley rats .
	manualset3
140121	3	408536	5	NULL	NULL	0	NULL	protovertarine B	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of protovertarines A and B , which stimulate carotid sinus baroreceptors and vagal sensory endings in the heart as well as pulmonary bed , were assessed on spontaneous and postsigh central sleep apneas in freely moving Sprague-Dawley rats .
	manualset3
140122	4	408536	5	NULL	NULL	0	NULL	carotid sinus baroreceptors	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of protovertarines A and B , which stimulate carotid sinus baroreceptors and vagal sensory endings in the heart as well as pulmonary bed , were assessed on spontaneous and postsigh central sleep apneas in freely moving Sprague-Dawley rats .
	manualset3
140123	5	408536	5	NULL	NULL	0	NULL	vagal sensory endings	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of protovertarines A and B , which stimulate carotid sinus baroreceptors and vagal sensory endings in the heart as well as pulmonary bed , were assessed on spontaneous and postsigh central sleep apneas in freely moving Sprague-Dawley rats .
	manualset3
140124	6	408536	5	NULL	NULL	0	NULL	heart 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of protovertarines A and B , which stimulate carotid sinus baroreceptors and vagal sensory endings in the heart as well as pulmonary bed , were assessed on spontaneous and postsigh central sleep apneas in freely moving Sprague-Dawley rats .
	manualset3
140125	7	408536	5	NULL	NULL	0	NULL	pulmonary bed	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of protovertarines A and B , which stimulate carotid sinus baroreceptors and vagal sensory endings in the heart as well as pulmonary bed , were assessed on spontaneous and postsigh central sleep apneas in freely moving Sprague-Dawley rats .
	manualset3
140126	8	408536	5	NULL	NULL	0	NULL	spontaneous and postsigh central sleep apneas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of protovertarines A and B , which stimulate carotid sinus baroreceptors and vagal sensory endings in the heart as well as pulmonary bed , were assessed on spontaneous and postsigh central sleep apneas in freely moving Sprague-Dawley rats .
	manualset3
140127	9	408536	5	NULL	NULL	0	NULL	Sprague-Dawley rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of protovertarines A and B , which stimulate carotid sinus baroreceptors and vagal sensory endings in the heart as well as pulmonary bed , were assessed on spontaneous and postsigh central sleep apneas in freely moving Sprague-Dawley rats .
	manualset3
140128	1	408537	5	NULL	NULL	0	NULL	action 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of quinidine interpreted from intracellular potentials of single cardiac fibers .
	manualset3
140129	2	408537	5	NULL	NULL	0	NULL	quinidine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of quinidine interpreted from intracellular potentials of single cardiac fibers .
	manualset3
140130	3	408537	5	NULL	NULL	0	NULL	intracellular potentials 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The action of quinidine interpreted from intracellular potentials of single cardiac fibers .
	manualset3
140131	4	408537	5	NULL	NULL	NULL	NULL	single cardiac fibers	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The action of quinidine interpreted from intracellular potentials of single cardiac fibers .
	manualset3
140132	1	408538	5	NULL	NULL	0	NULL	actions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The actions of ( + ) - catechin on cell-induced oxidation of LDL are consistent with the ability of flavonoids of similar structure to inhibit lipoxygenases and with a role for lipoxygenases in cell-induced modification of LDL in vivo .
	manualset3
140133	2	408538	5	NULL	NULL	0	NULL	( + ) - catechin	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The actions of ( + ) - catechin on cell-induced oxidation of LDL are consistent with the ability of flavonoids of similar structure to inhibit lipoxygenases and with a role for lipoxygenases in cell-induced modification of LDL in vivo .
	manualset3
140134	3	408538	5	NULL	NULL	NULL	NULL	cell-induced oxidation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The actions of ( + ) - catechin on cell-induced oxidation of LDL are consistent with the ability of flavonoids of similar structure to inhibit lipoxygenases and with a role for lipoxygenases in cell-induced modification of LDL in vivo .
	manualset3
140135	4	408538	5	NULL	NULL	0	NULL	LDL	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The actions of ( + ) - catechin on cell-induced oxidation of LDL are consistent with the ability of flavonoids of similar structure to inhibit lipoxygenases and with a role for lipoxygenases in cell-induced modification of LDL in vivo .
	manualset3
140136	5	408538	5	NULL	NULL	0	NULL	ability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The actions of ( + ) - catechin on cell-induced oxidation of LDL are consistent with the ability of flavonoids of similar structure to inhibit lipoxygenases and with a role for lipoxygenases in cell-induced modification of LDL in vivo .
	manualset3
140137	6	408538	5	NULL	NULL	0	NULL	flavonoids 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The actions of ( + ) - catechin on cell-induced oxidation of LDL are consistent with the ability of flavonoids of similar structure to inhibit lipoxygenases and with a role for lipoxygenases in cell-induced modification of LDL in vivo .
	manualset3
140138	7	408538	5	NULL	NULL	0	NULL	structure 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The actions of ( + ) - catechin on cell-induced oxidation of LDL are consistent with the ability of flavonoids of similar structure to inhibit lipoxygenases and with a role for lipoxygenases in cell-induced modification of LDL in vivo .
	manualset3
140139	8	408538	5	NULL	NULL	0	NULL	lipoxygenases 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The actions of ( + ) - catechin on cell-induced oxidation of LDL are consistent with the ability of flavonoids of similar structure to inhibit lipoxygenases and with a role for lipoxygenases in cell-induced modification of LDL in vivo .
	manualset3
140140	9	408538	5	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The actions of ( + ) - catechin on cell-induced oxidation of LDL are consistent with the ability of flavonoids of similar structure to inhibit lipoxygenases and with a role for lipoxygenases in cell-induced modification of LDL in vivo .
	manualset3
140141	10	408538	5	NULL	NULL	0	NULL	lipoxygenases 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The actions of ( + ) - catechin on cell-induced oxidation of LDL are consistent with the ability of flavonoids of similar structure to inhibit lipoxygenases and with a role for lipoxygenases in cell-induced modification of LDL in vivo .
	manualset3
140142	11	408538	5	NULL	NULL	0	NULL	cell-induced modification 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The actions of ( + ) - catechin on cell-induced oxidation of LDL are consistent with the ability of flavonoids of similar structure to inhibit lipoxygenases and with a role for lipoxygenases in cell-induced modification of LDL in vivo .
	manualset3
140143	12	408538	5	NULL	NULL	0	NULL	LDL 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The actions of ( + ) - catechin on cell-induced oxidation of LDL are consistent with the ability of flavonoids of similar structure to inhibit lipoxygenases and with a role for lipoxygenases in cell-induced modification of LDL in vivo .
	manualset3
140144	1	408539	5	NULL	NULL	0	NULL	actions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The actions of benzodiazepines and pentobarbitone on GABA-mediated recurrent inhibition of hippocampal pyramidal neurons were investigated in the immobilized unanaesthetized cat .
	manualset3
140145	2	408539	5	NULL	NULL	0	NULL	benzodiazepines 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The actions of benzodiazepines and pentobarbitone on GABA-mediated recurrent inhibition of hippocampal pyramidal neurons were investigated in the immobilized unanaesthetized cat .
	manualset3
140146	3	408539	5	NULL	NULL	0	NULL	pentobarbitone 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The actions of benzodiazepines and pentobarbitone on GABA-mediated recurrent inhibition of hippocampal pyramidal neurons were investigated in the immobilized unanaesthetized cat .
	manualset3
140147	4	408539	5	NULL	NULL	0	NULL	GABA-mediated recurrent inhibition 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The actions of benzodiazepines and pentobarbitone on GABA-mediated recurrent inhibition of hippocampal pyramidal neurons were investigated in the immobilized unanaesthetized cat .
	manualset3
140148	5	408539	5	NULL	NULL	0	NULL	hippocampal pyramidal neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The actions of benzodiazepines and pentobarbitone on GABA-mediated recurrent inhibition of hippocampal pyramidal neurons were investigated in the immobilized unanaesthetized cat .
	manualset3
140149	6	408539	5	NULL	NULL	0	NULL	unanaesthetized cat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The actions of benzodiazepines and pentobarbitone on GABA-mediated recurrent inhibition of hippocampal pyramidal neurons were investigated in the immobilized unanaesthetized cat .
	manualset3
140150	1	408540	5	NULL	NULL	0	NULL	actions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The actions of one atrium with a frequency of 55 -- 60/minute were transmitted regularly to the ventricles ; the actions of the other atrium had a frequency of 90/minute and were not transmitted .
	manualset3
140151	2	408540	5	NULL	NULL	0	NULL	one 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The actions of one atrium with a frequency of 55 -- 60/minute were transmitted regularly to the ventricles ; the actions of the other atrium had a frequency of 90/minute and were not transmitted .
	manualset3
140152	3	408540	5	NULL	NULL	0	NULL	atrium 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The actions of one atrium with a frequency of 55 -- 60/minute were transmitted regularly to the ventricles ; the actions of the other atrium had a frequency of 90/minute and were not transmitted .
	manualset3
140153	4	408540	5	NULL	NULL	0	NULL	frequency 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The actions of one atrium with a frequency of 55 -- 60/minute were transmitted regularly to the ventricles ; the actions of the other atrium had a frequency of 90/minute and were not transmitted .
	manualset3
140154	5	408540	5	NULL	NULL	0	NULL	55 -- 60/minute 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The actions of one atrium with a frequency of 55 -- 60/minute were transmitted regularly to the ventricles ; the actions of the other atrium had a frequency of 90/minute and were not transmitted .
	manualset3
140155	6	408540	5	NULL	NULL	0	NULL	ventricles 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The actions of one atrium with a frequency of 55 -- 60/minute were transmitted regularly to the ventricles ; the actions of the other atrium had a frequency of 90/minute and were not transmitted .
	manualset3
140156	7	408540	5	NULL	NULL	0	NULL	actions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The actions of one atrium with a frequency of 55 -- 60/minute were transmitted regularly to the ventricles ; the actions of the other atrium had a frequency of 90/minute and were not transmitted .
	manualset3
140157	8	408540	5	NULL	NULL	0	NULL	atrium 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The actions of one atrium with a frequency of 55 -- 60/minute were transmitted regularly to the ventricles ; the actions of the other atrium had a frequency of 90/minute and were not transmitted .
	manualset3
140158	9	408540	5	NULL	NULL	0	NULL	frequency 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The actions of one atrium with a frequency of 55 -- 60/minute were transmitted regularly to the ventricles ; the actions of the other atrium had a frequency of 90/minute and were not transmitted .
	manualset3
140159	10	408540	5	NULL	NULL	0	NULL	90/minute	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The actions of one atrium with a frequency of 55 -- 60/minute were transmitted regularly to the ventricles ; the actions of the other atrium had a frequency of 90/minute and were not transmitted .
	manualset3
140160	1	408541	5	NULL	NULL	0	NULL	activation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation , as in the case of trypsinogen , takes place only in an acid medium .
	manualset3
140161	2	408541	5	NULL	NULL	0	NULL	case 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation , as in the case of trypsinogen , takes place only in an acid medium .
	manualset3
140162	3	408541	5	NULL	NULL	0	NULL	trypsinogen 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation , as in the case of trypsinogen , takes place only in an acid medium .
	manualset3
140163	4	408541	5	NULL	NULL	0	NULL	acid medium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation , as in the case of trypsinogen , takes place only in an acid medium .
	manualset3
140164	1	408542	5	NULL	NULL	0	NULL	activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation of Proteinase-Activated Receptor-1 ( PAR1 ) mediates gastric cancer cell proliferation and invasion .
	manualset3
140165	2	408542	5	NULL	NULL	0	NULL	Proteinase-Activated Receptor-1 ( PAR1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation of Proteinase-Activated Receptor-1 ( PAR1 ) mediates gastric cancer cell proliferation and invasion .
	manualset3
140166	3	408542	5	NULL	NULL	0	NULL	gastric cancer cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation of Proteinase-Activated Receptor-1 ( PAR1 ) mediates gastric cancer cell proliferation and invasion .
	manualset3
140167	4	408542	5	NULL	NULL	0	NULL	invasion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation of Proteinase-Activated Receptor-1 ( PAR1 ) mediates gastric cancer cell proliferation and invasion .
	manualset3
140168	1	408543	5	NULL	NULL	0	NULL	activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation of beta-catenin promotes extracellular signal-related kinase ( ERK ) phosphorylation , resulting in the increased expression of antiapoptotic protein B-cell leukemia 2 ( Bcl-2 ) , which may contribute to the maintenance of NK-cell survival .
	manualset3
140169	2	408543	5	NULL	NULL	0	NULL	beta-catenin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation of beta-catenin promotes extracellular signal-related kinase ( ERK ) phosphorylation , resulting in the increased expression of antiapoptotic protein B-cell leukemia 2 ( Bcl-2 ) , which may contribute to the maintenance of NK-cell survival .
	manualset3
140170	3	408543	5	NULL	NULL	0	NULL	extracellular signal-related kinase ( ERK ) phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation of beta-catenin promotes extracellular signal-related kinase ( ERK ) phosphorylation , resulting in the increased expression of antiapoptotic protein B-cell leukemia 2 ( Bcl-2 ) , which may contribute to the maintenance of NK-cell survival .
	manualset3
140171	4	408543	5	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation of beta-catenin promotes extracellular signal-related kinase ( ERK ) phosphorylation , resulting in the increased expression of antiapoptotic protein B-cell leukemia 2 ( Bcl-2 ) , which may contribute to the maintenance of NK-cell survival .
	manualset3
140172	5	408543	5	NULL	NULL	0	NULL	antiapoptotic protein B-cell leukemia 2 ( Bcl-2 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation of beta-catenin promotes extracellular signal-related kinase ( ERK ) phosphorylation , resulting in the increased expression of antiapoptotic protein B-cell leukemia 2 ( Bcl-2 ) , which may contribute to the maintenance of NK-cell survival .
	manualset3
140173	6	408543	5	NULL	NULL	0	NULL	maintenance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation of beta-catenin promotes extracellular signal-related kinase ( ERK ) phosphorylation , resulting in the increased expression of antiapoptotic protein B-cell leukemia 2 ( Bcl-2 ) , which may contribute to the maintenance of NK-cell survival .
	manualset3
140174	7	408543	5	NULL	NULL	0	NULL	NK-cell survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation of beta-catenin promotes extracellular signal-related kinase ( ERK ) phosphorylation , resulting in the increased expression of antiapoptotic protein B-cell leukemia 2 ( Bcl-2 ) , which may contribute to the maintenance of NK-cell survival .
	manualset3
140175	1	408544	5	NULL	NULL	0	NULL	activation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation of human platelets is inhibited by two intracellular pathways regulated by either cGMP - or cAMP-elevating agents .
	manualset3
140176	2	408544	5	NULL	NULL	0	NULL	human platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation of human platelets is inhibited by two intracellular pathways regulated by either cGMP - or cAMP-elevating agents .
	manualset3
140177	3	408544	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation of human platelets is inhibited by two intracellular pathways regulated by either cGMP - or cAMP-elevating agents .
	manualset3
140178	4	408544	5	NULL	NULL	0	NULL	intracellular pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation of human platelets is inhibited by two intracellular pathways regulated by either cGMP - or cAMP-elevating agents .
	manualset3
140179	5	408544	5	NULL	NULL	0	NULL	cGMP - elevating agents	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation of human platelets is inhibited by two intracellular pathways regulated by either cGMP - or cAMP-elevating agents .
	manualset3
140180	6	408544	5	NULL	NULL	0	NULL	cAMP-elevating agents	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation of human platelets is inhibited by two intracellular pathways regulated by either cGMP - or cAMP-elevating agents .
	manualset3
140181	1	408545	5	NULL	NULL	0	NULL	activation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation of macrophages by malarial GPIs involves engagement of Toll like receptor 2 ( TLR2 ) resulting in the intracellular signaling and production of cytokines .
	manualset3
140182	2	408545	5	NULL	NULL	0	NULL	macrophages 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation of macrophages by malarial GPIs involves engagement of Toll like receptor 2 ( TLR2 ) resulting in the intracellular signaling and production of cytokines .
	manualset3
140183	3	408545	5	NULL	NULL	0	NULL	malarial GPIs	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation of macrophages by malarial GPIs involves engagement of Toll like receptor 2 ( TLR2 ) resulting in the intracellular signaling and production of cytokines .
	manualset3
140184	4	408545	5	NULL	NULL	0	NULL	engagement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation of macrophages by malarial GPIs involves engagement of Toll like receptor 2 ( TLR2 ) resulting in the intracellular signaling and production of cytokines .
	manualset3
140185	5	408545	5	NULL	NULL	0	NULL	Toll like receptor 2 ( TLR2 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation of macrophages by malarial GPIs involves engagement of Toll like receptor 2 ( TLR2 ) resulting in the intracellular signaling and production of cytokines .
	manualset3
140186	6	408545	5	NULL	NULL	0	NULL	intracellular signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation of macrophages by malarial GPIs involves engagement of Toll like receptor 2 ( TLR2 ) resulting in the intracellular signaling and production of cytokines .
	manualset3
140187	7	408545	5	NULL	NULL	0	NULL	production of cytokines	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation of macrophages by malarial GPIs involves engagement of Toll like receptor 2 ( TLR2 ) resulting in the intracellular signaling and production of cytokines .
	manualset3
140188	1	408546	5	NULL	NULL	0	NULL	activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation of stress kinases by hyperosmolarity occurs independent of the IR .
	manualset3
140189	2	408546	5	NULL	NULL	0	NULL	stress kinases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation of stress kinases by hyperosmolarity occurs independent of the IR .
	manualset3
140190	3	408546	5	NULL	NULL	0	NULL	hyperosmolarity 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation of stress kinases by hyperosmolarity occurs independent of the IR .
	manualset3
140191	4	408546	5	NULL	NULL	0	NULL	 IR	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The activation of stress kinases by hyperosmolarity occurs independent of the IR .
	manualset3
140192	1	408547	5	NULL	NULL	0	NULL	active component	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The active component of the extract was identified as the glucoside of salicylic alcohol .
	manualset3
140193	2	408547	5	NULL	NULL	0	NULL	extract 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The active component of the extract was identified as the glucoside of salicylic alcohol .
	manualset3
140194	3	408547	5	NULL	NULL	0	NULL	glucoside 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The active component of the extract was identified as the glucoside of salicylic alcohol .
	manualset3
140195	4	408547	5	NULL	NULL	0	NULL	salicylic alcohol	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The active component of the extract was identified as the glucoside of salicylic alcohol .
	manualset3
140196	1	408548	5	NULL	NULL	0	NULL	activities 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The activities of cytidine triphosphate synthetase , deoxycytidine monophosphate deaminase , uridine kinase , thymidine kinase , thymidine monophosphate kinase and DNA polymerase were markedly increased in tumor tissues , compared with those in the corresponding normal tissues , while the activities of deoxycytidine kinase , cytidine deaminase and deoxycytidine deaminase were only slightly increased .
	manualset3
140197	2	408548	5	NULL	NULL	0	NULL	cytidine triphosphate synthetase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The activities of cytidine triphosphate synthetase , deoxycytidine monophosphate deaminase , uridine kinase , thymidine kinase , thymidine monophosphate kinase and DNA polymerase were markedly increased in tumor tissues , compared with those in the corresponding normal tissues , while the activities of deoxycytidine kinase , cytidine deaminase and deoxycytidine deaminase were only slightly increased .
	manualset3
140198	3	408548	5	NULL	NULL	0	NULL	deoxycytidine monophosphate deaminase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The activities of cytidine triphosphate synthetase , deoxycytidine monophosphate deaminase , uridine kinase , thymidine kinase , thymidine monophosphate kinase and DNA polymerase were markedly increased in tumor tissues , compared with those in the corresponding normal tissues , while the activities of deoxycytidine kinase , cytidine deaminase and deoxycytidine deaminase were only slightly increased .
	manualset3
140199	4	408548	5	NULL	NULL	0	NULL	uridine kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The activities of cytidine triphosphate synthetase , deoxycytidine monophosphate deaminase , uridine kinase , thymidine kinase , thymidine monophosphate kinase and DNA polymerase were markedly increased in tumor tissues , compared with those in the corresponding normal tissues , while the activities of deoxycytidine kinase , cytidine deaminase and deoxycytidine deaminase were only slightly increased .
	manualset3
140200	5	408548	5	NULL	NULL	0	NULL	thymidine kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The activities of cytidine triphosphate synthetase , deoxycytidine monophosphate deaminase , uridine kinase , thymidine kinase , thymidine monophosphate kinase and DNA polymerase were markedly increased in tumor tissues , compared with those in the corresponding normal tissues , while the activities of deoxycytidine kinase , cytidine deaminase and deoxycytidine deaminase were only slightly increased .
	manualset3
140201	6	408548	5	NULL	NULL	0	NULL	thymidine monophosphate kinase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The activities of cytidine triphosphate synthetase , deoxycytidine monophosphate deaminase , uridine kinase , thymidine kinase , thymidine monophosphate kinase and DNA polymerase were markedly increased in tumor tissues , compared with those in the corresponding normal tissues , while the activities of deoxycytidine kinase , cytidine deaminase and deoxycytidine deaminase were only slightly increased .
	manualset3
140202	7	408548	5	NULL	NULL	0	NULL	DNA polymerase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The activities of cytidine triphosphate synthetase , deoxycytidine monophosphate deaminase , uridine kinase , thymidine kinase , thymidine monophosphate kinase and DNA polymerase were markedly increased in tumor tissues , compared with those in the corresponding normal tissues , while the activities of deoxycytidine kinase , cytidine deaminase and deoxycytidine deaminase were only slightly increased .
	manualset3
140203	8	408548	5	NULL	NULL	0	NULL	tumor tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The activities of cytidine triphosphate synthetase , deoxycytidine monophosphate deaminase , uridine kinase , thymidine kinase , thymidine monophosphate kinase and DNA polymerase were markedly increased in tumor tissues , compared with those in the corresponding normal tissues , while the activities of deoxycytidine kinase , cytidine deaminase and deoxycytidine deaminase were only slightly increased .
	manualset3
140204	9	408548	5	NULL	NULL	0	NULL	normal tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The activities of cytidine triphosphate synthetase , deoxycytidine monophosphate deaminase , uridine kinase , thymidine kinase , thymidine monophosphate kinase and DNA polymerase were markedly increased in tumor tissues , compared with those in the corresponding normal tissues , while the activities of deoxycytidine kinase , cytidine deaminase and deoxycytidine deaminase were only slightly increased .
	manualset3
140205	10	408548	5	NULL	NULL	0	NULL	activities 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The activities of cytidine triphosphate synthetase , deoxycytidine monophosphate deaminase , uridine kinase , thymidine kinase , thymidine monophosphate kinase and DNA polymerase were markedly increased in tumor tissues , compared with those in the corresponding normal tissues , while the activities of deoxycytidine kinase , cytidine deaminase and deoxycytidine deaminase were only slightly increased .
	manualset3
140206	11	408548	5	NULL	NULL	0	NULL	deoxycytidine kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The activities of cytidine triphosphate synthetase , deoxycytidine monophosphate deaminase , uridine kinase , thymidine kinase , thymidine monophosphate kinase and DNA polymerase were markedly increased in tumor tissues , compared with those in the corresponding normal tissues , while the activities of deoxycytidine kinase , cytidine deaminase and deoxycytidine deaminase were only slightly increased .
	manualset3
140207	12	408548	5	NULL	NULL	0	NULL	cytidine deaminase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The activities of cytidine triphosphate synthetase , deoxycytidine monophosphate deaminase , uridine kinase , thymidine kinase , thymidine monophosphate kinase and DNA polymerase were markedly increased in tumor tissues , compared with those in the corresponding normal tissues , while the activities of deoxycytidine kinase , cytidine deaminase and deoxycytidine deaminase were only slightly increased .
	manualset3
140208	13	408548	5	NULL	NULL	0	NULL	deoxycytidine deaminase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The activities of cytidine triphosphate synthetase , deoxycytidine monophosphate deaminase , uridine kinase , thymidine kinase , thymidine monophosphate kinase and DNA polymerase were markedly increased in tumor tissues , compared with those in the corresponding normal tissues , while the activities of deoxycytidine kinase , cytidine deaminase and deoxycytidine deaminase were only slightly increased .
	manualset3
140209	1	408549	5	NULL	NULL	0	NULL	activities 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The activities of the salt-sensitive peptide P-113 were diminished at high salt concentrations , whereas the activities of its - naphthylalanine and - ( 4 , 4 ' - biphenyl ) alanine-substituted variant were less affected .
	manualset3
140210	2	408549	5	NULL	NULL	0	NULL	salt-sensitive peptide P-113	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The activities of the salt-sensitive peptide P-113 were diminished at high salt concentrations , whereas the activities of its - naphthylalanine and - ( 4 , 4 ' - biphenyl ) alanine-substituted variant were less affected .
	manualset3
140211	3	408549	5	NULL	NULL	0	NULL	high salt concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The activities of the salt-sensitive peptide P-113 were diminished at high salt concentrations , whereas the activities of its - naphthylalanine and - ( 4 , 4 ' - biphenyl ) alanine-substituted variant were less affected .
	manualset3
140212	4	408549	5	NULL	NULL	0	NULL	activities 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The activities of the salt-sensitive peptide P-113 were diminished at high salt concentrations , whereas the activities of its - naphthylalanine and - ( 4 , 4 ' - biphenyl ) alanine-substituted variant were less affected .
	manualset3
140213	5	408549	5	NULL	NULL	NULL	NULL	naphthylalanine substituted variant 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The activities of the salt-sensitive peptide P-113 were diminished at high salt concentrations , whereas the activities of its - naphthylalanine and - ( 4 , 4 ' - biphenyl ) alanine-substituted variant were less affected .
	manualset3
140214	6	408549	5	NULL	NULL	0	NULL	( 4 , 4 ' - biphenyl ) alanine-substituted variant	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The activities of the salt-sensitive peptide P-113 were diminished at high salt concentrations , whereas the activities of its - naphthylalanine and - ( 4 , 4 ' - biphenyl ) alanine-substituted variant were less affected .
	manualset3
140215	1	408550	5	NULL	NULL	0	NULL	activity levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity levels of pyruvate dehydrogenase , enzymes of the citric acid cycle , aspartate and alanine aminotransferases , and NADP + - isocitrate dehydrogenase were determined in the cerebral cortex , cerebellum , brain stem , corpus striatum , hippocampus , and midbrain regions of normal rats and rats injected with acute and subacute doses of methionine sulfoximine ( MSI ) .
	manualset3
140216	2	408550	5	NULL	NULL	0	NULL	pyruvate dehydrogenase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity levels of pyruvate dehydrogenase , enzymes of the citric acid cycle , aspartate and alanine aminotransferases , and NADP + - isocitrate dehydrogenase were determined in the cerebral cortex , cerebellum , brain stem , corpus striatum , hippocampus , and midbrain regions of normal rats and rats injected with acute and subacute doses of methionine sulfoximine ( MSI ) .
	manualset3
140217	3	408550	5	NULL	NULL	0	NULL	enzymes of the citric acid cycle 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity levels of pyruvate dehydrogenase , enzymes of the citric acid cycle , aspartate and alanine aminotransferases , and NADP + - isocitrate dehydrogenase were determined in the cerebral cortex , cerebellum , brain stem , corpus striatum , hippocampus , and midbrain regions of normal rats and rats injected with acute and subacute doses of methionine sulfoximine ( MSI ) .
	manualset3
140218	4	408550	5	NULL	NULL	0	NULL	aspartate aminotransferases 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity levels of pyruvate dehydrogenase , enzymes of the citric acid cycle , aspartate and alanine aminotransferases , and NADP + - isocitrate dehydrogenase were determined in the cerebral cortex , cerebellum , brain stem , corpus striatum , hippocampus , and midbrain regions of normal rats and rats injected with acute and subacute doses of methionine sulfoximine ( MSI ) .
	manualset3
140219	5	408550	5	NULL	NULL	0	NULL	alanine aminotransferases 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity levels of pyruvate dehydrogenase , enzymes of the citric acid cycle , aspartate and alanine aminotransferases , and NADP + - isocitrate dehydrogenase were determined in the cerebral cortex , cerebellum , brain stem , corpus striatum , hippocampus , and midbrain regions of normal rats and rats injected with acute and subacute doses of methionine sulfoximine ( MSI ) .
	manualset3
140220	6	408550	5	NULL	NULL	0	NULL	NADP + - isocitrate dehydrogenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity levels of pyruvate dehydrogenase , enzymes of the citric acid cycle , aspartate and alanine aminotransferases , and NADP + - isocitrate dehydrogenase were determined in the cerebral cortex , cerebellum , brain stem , corpus striatum , hippocampus , and midbrain regions of normal rats and rats injected with acute and subacute doses of methionine sulfoximine ( MSI ) .
	manualset3
140221	7	408550	5	NULL	NULL	0	NULL	cerebral cortex 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity levels of pyruvate dehydrogenase , enzymes of the citric acid cycle , aspartate and alanine aminotransferases , and NADP + - isocitrate dehydrogenase were determined in the cerebral cortex , cerebellum , brain stem , corpus striatum , hippocampus , and midbrain regions of normal rats and rats injected with acute and subacute doses of methionine sulfoximine ( MSI ) .
	manualset3
140222	8	408550	5	NULL	NULL	0	NULL	cerebellum 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity levels of pyruvate dehydrogenase , enzymes of the citric acid cycle , aspartate and alanine aminotransferases , and NADP + - isocitrate dehydrogenase were determined in the cerebral cortex , cerebellum , brain stem , corpus striatum , hippocampus , and midbrain regions of normal rats and rats injected with acute and subacute doses of methionine sulfoximine ( MSI ) .
	manualset3
140223	9	408550	5	NULL	NULL	0	NULL	brain stem	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity levels of pyruvate dehydrogenase , enzymes of the citric acid cycle , aspartate and alanine aminotransferases , and NADP + - isocitrate dehydrogenase were determined in the cerebral cortex , cerebellum , brain stem , corpus striatum , hippocampus , and midbrain regions of normal rats and rats injected with acute and subacute doses of methionine sulfoximine ( MSI ) .
	manualset3
140224	10	408550	5	NULL	NULL	0	NULL	corpus striatum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity levels of pyruvate dehydrogenase , enzymes of the citric acid cycle , aspartate and alanine aminotransferases , and NADP + - isocitrate dehydrogenase were determined in the cerebral cortex , cerebellum , brain stem , corpus striatum , hippocampus , and midbrain regions of normal rats and rats injected with acute and subacute doses of methionine sulfoximine ( MSI ) .
	manualset3
140225	11	408550	5	NULL	NULL	0	NULL	hippocampus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity levels of pyruvate dehydrogenase , enzymes of the citric acid cycle , aspartate and alanine aminotransferases , and NADP + - isocitrate dehydrogenase were determined in the cerebral cortex , cerebellum , brain stem , corpus striatum , hippocampus , and midbrain regions of normal rats and rats injected with acute and subacute doses of methionine sulfoximine ( MSI ) .
	manualset3
140226	12	408550	5	NULL	NULL	0	NULL	midbrain regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity levels of pyruvate dehydrogenase , enzymes of the citric acid cycle , aspartate and alanine aminotransferases , and NADP + - isocitrate dehydrogenase were determined in the cerebral cortex , cerebellum , brain stem , corpus striatum , hippocampus , and midbrain regions of normal rats and rats injected with acute and subacute doses of methionine sulfoximine ( MSI ) .
	manualset3
140227	13	408550	5	NULL	NULL	0	NULL	normal rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity levels of pyruvate dehydrogenase , enzymes of the citric acid cycle , aspartate and alanine aminotransferases , and NADP + - isocitrate dehydrogenase were determined in the cerebral cortex , cerebellum , brain stem , corpus striatum , hippocampus , and midbrain regions of normal rats and rats injected with acute and subacute doses of methionine sulfoximine ( MSI ) .
	manualset3
140228	14	408550	5	NULL	NULL	0	NULL	rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity levels of pyruvate dehydrogenase , enzymes of the citric acid cycle , aspartate and alanine aminotransferases , and NADP + - isocitrate dehydrogenase were determined in the cerebral cortex , cerebellum , brain stem , corpus striatum , hippocampus , and midbrain regions of normal rats and rats injected with acute and subacute doses of methionine sulfoximine ( MSI ) .
	manualset3
140229	15	408550	5	NULL	NULL	0	NULL	acute doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity levels of pyruvate dehydrogenase , enzymes of the citric acid cycle , aspartate and alanine aminotransferases , and NADP + - isocitrate dehydrogenase were determined in the cerebral cortex , cerebellum , brain stem , corpus striatum , hippocampus , and midbrain regions of normal rats and rats injected with acute and subacute doses of methionine sulfoximine ( MSI ) .
	manualset3
140230	16	408550	5	NULL	NULL	0	NULL	subacute doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity levels of pyruvate dehydrogenase , enzymes of the citric acid cycle , aspartate and alanine aminotransferases , and NADP + - isocitrate dehydrogenase were determined in the cerebral cortex , cerebellum , brain stem , corpus striatum , hippocampus , and midbrain regions of normal rats and rats injected with acute and subacute doses of methionine sulfoximine ( MSI ) .
	manualset3
140231	17	408550	5	NULL	NULL	0	NULL	methionine sulfoximine ( MSI ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity levels of pyruvate dehydrogenase , enzymes of the citric acid cycle , aspartate and alanine aminotransferases , and NADP + - isocitrate dehydrogenase were determined in the cerebral cortex , cerebellum , brain stem , corpus striatum , hippocampus , and midbrain regions of normal rats and rats injected with acute and subacute doses of methionine sulfoximine ( MSI ) .
	manualset3
140232	1	408551	5	NULL	NULL	0	NULL	activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of DVF-B decrease markedly at pH 6.0 but was stable at pH 6.5 to 8.5 .
	manualset3
140233	2	408551	5	NULL	NULL	0	NULL	DVF-B	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of DVF-B decrease markedly at pH 6.0 but was stable at pH 6.5 to 8.5 .
	manualset3
140234	3	408551	5	NULL	NULL	0	NULL	pH 6.0 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of DVF-B decrease markedly at pH 6.0 but was stable at pH 6.5 to 8.5 .
	manualset3
140235	4	408551	5	NULL	NULL	0	NULL	 pH 6.5 to 8.5	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of DVF-B decrease markedly at pH 6.0 but was stable at pH 6.5 to 8.5 .
	manualset3
140236	1	408552	5	NULL	NULL	0	NULL	Chemica damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Chemica damage to the eye in industrial medicine ) .
	manualset3
140237	2	408552	5	NULL	NULL	0	NULL	eye 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Chemica damage to the eye in industrial medicine ) .
	manualset3
140238	3	408552	5	NULL	NULL	0	NULL	industrial medicine	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Chemica damage to the eye in industrial medicine ) .
	manualset3
140239	1	408553	5	NULL	NULL	0	NULL	activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of c-Jun NH ( 2 ) - terminal kinase was gonadal hormone-independent .
	manualset3
140240	2	408553	5	NULL	NULL	0	NULL	c-Jun NH ( 2 ) - terminal kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of c-Jun NH ( 2 ) - terminal kinase was gonadal hormone-independent .
	manualset3
140241	1	408554	5	NULL	NULL	0	NULL	activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of gamma-aminobutyrate aminotransferase ( GABA-T ) was estimated in twelve regions of brains from 22 control subjects and 6 cases with schizophrenia .
	manualset3
140242	2	408554	5	NULL	NULL	0	NULL	gamma-aminobutyrate aminotransferase ( GABA-T )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of gamma-aminobutyrate aminotransferase ( GABA-T ) was estimated in twelve regions of brains from 22 control subjects and 6 cases with schizophrenia .
	manualset3
140243	3	408554	5	NULL	NULL	0	NULL	twelve regions of brains	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of gamma-aminobutyrate aminotransferase ( GABA-T ) was estimated in twelve regions of brains from 22 control subjects and 6 cases with schizophrenia .
	manualset3
140244	4	408554	5	NULL	NULL	0	NULL	22	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of gamma-aminobutyrate aminotransferase ( GABA-T ) was estimated in twelve regions of brains from 22 control subjects and 6 cases with schizophrenia .
	manualset3
140245	5	408554	5	NULL	NULL	0	NULL	control subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of gamma-aminobutyrate aminotransferase ( GABA-T ) was estimated in twelve regions of brains from 22 control subjects and 6 cases with schizophrenia .
	manualset3
140246	6	408554	5	NULL	NULL	0	NULL	6 cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of gamma-aminobutyrate aminotransferase ( GABA-T ) was estimated in twelve regions of brains from 22 control subjects and 6 cases with schizophrenia .
	manualset3
140247	7	408554	5	NULL	NULL	0	NULL	schizophrenia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of gamma-aminobutyrate aminotransferase ( GABA-T ) was estimated in twelve regions of brains from 22 control subjects and 6 cases with schizophrenia .
	manualset3
140248	1	408555	5	NULL	NULL	0	NULL	activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of glutathione peroxidase was higher in the selenium-treated group than in the animals that were irradiated but received no treatment .
	manualset3
140249	2	408555	5	NULL	NULL	0	NULL	glutathione peroxidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of glutathione peroxidase was higher in the selenium-treated group than in the animals that were irradiated but received no treatment .
	manualset3
140250	3	408555	5	NULL	NULL	0	NULL	selenium-treated group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of glutathione peroxidase was higher in the selenium-treated group than in the animals that were irradiated but received no treatment .
	manualset3
140251	4	408555	5	NULL	NULL	0	NULL	animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of glutathione peroxidase was higher in the selenium-treated group than in the animals that were irradiated but received no treatment .
	manualset3
140252	5	408555	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of glutathione peroxidase was higher in the selenium-treated group than in the animals that were irradiated but received no treatment .
	manualset3
140253	1	408556	5	NULL	NULL	0	NULL	activity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of rats in a swimming situation as a function of water temperature .
	manualset3
140254	2	408556	5	NULL	NULL	0	NULL	rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of rats in a swimming situation as a function of water temperature .
	manualset3
140255	3	408556	5	NULL	NULL	0	NULL	swimming situation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of rats in a swimming situation as a function of water temperature .
	manualset3
140256	4	408556	5	NULL	NULL	0	NULL	function 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of rats in a swimming situation as a function of water temperature .
	manualset3
140257	5	408556	5	NULL	NULL	0	NULL	water temperature	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of rats in a swimming situation as a function of water temperature .
	manualset3
140258	1	408557	5	NULL	NULL	0	NULL	activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of succinate dehydrogenase ( SDH ) in lymphocytes of peripheral blood of AKR mice was measured in response to intraperitoneal injection of epinephrine hydrochloride at a dose of 1 mg/kg .
	manualset3
140259	2	408557	5	NULL	NULL	0	NULL	succinate dehydrogenase ( SDH )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of succinate dehydrogenase ( SDH ) in lymphocytes of peripheral blood of AKR mice was measured in response to intraperitoneal injection of epinephrine hydrochloride at a dose of 1 mg/kg .
	manualset3
140260	3	408557	5	NULL	NULL	0	NULL	lymphocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of succinate dehydrogenase ( SDH ) in lymphocytes of peripheral blood of AKR mice was measured in response to intraperitoneal injection of epinephrine hydrochloride at a dose of 1 mg/kg .
	manualset3
140261	4	408557	5	NULL	NULL	0	NULL	peripheral blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of succinate dehydrogenase ( SDH ) in lymphocytes of peripheral blood of AKR mice was measured in response to intraperitoneal injection of epinephrine hydrochloride at a dose of 1 mg/kg .
	manualset3
140262	5	408557	5	NULL	NULL	0	NULL	AKR mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of succinate dehydrogenase ( SDH ) in lymphocytes of peripheral blood of AKR mice was measured in response to intraperitoneal injection of epinephrine hydrochloride at a dose of 1 mg/kg .
	manualset3
140263	6	408557	5	NULL	NULL	0	NULL	response 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of succinate dehydrogenase ( SDH ) in lymphocytes of peripheral blood of AKR mice was measured in response to intraperitoneal injection of epinephrine hydrochloride at a dose of 1 mg/kg .
	manualset3
140264	7	408557	5	NULL	NULL	0	NULL	intraperitoneal injection 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of succinate dehydrogenase ( SDH ) in lymphocytes of peripheral blood of AKR mice was measured in response to intraperitoneal injection of epinephrine hydrochloride at a dose of 1 mg/kg .
	manualset3
140265	8	408557	5	NULL	NULL	0	NULL	epinephrine hydrochloride	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of succinate dehydrogenase ( SDH ) in lymphocytes of peripheral blood of AKR mice was measured in response to intraperitoneal injection of epinephrine hydrochloride at a dose of 1 mg/kg .
	manualset3
140266	9	408557	5	NULL	NULL	0	NULL	dose 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of succinate dehydrogenase ( SDH ) in lymphocytes of peripheral blood of AKR mice was measured in response to intraperitoneal injection of epinephrine hydrochloride at a dose of 1 mg/kg .
	manualset3
140267	10	408557	5	NULL	NULL	0	NULL	1 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of succinate dehydrogenase ( SDH ) in lymphocytes of peripheral blood of AKR mice was measured in response to intraperitoneal injection of epinephrine hydrochloride at a dose of 1 mg/kg .
	manualset3
140268	1	408558	5	NULL	NULL	0	NULL	activity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of the bone and soft tissue tumor study group of the Japan clinical oncology group .
	manualset3
140269	2	408558	5	NULL	NULL	NULL	NULL	bone and soft tissue tumor study group 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The activity of the bone and soft tissue tumor study group of the Japan clinical oncology group .
	manualset3
140270	3	408558	5	NULL	NULL	0	NULL	Japan clinical oncology group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of the bone and soft tissue tumor study group of the Japan clinical oncology group .
	manualset3
140271	1	408559	5	NULL	NULL	0	NULL	activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of the mitochondrial - ketoglutarate dehydrogenase complex ( KGDHC ) in homogenates from autopsy brain declines with AD .
	manualset3
140272	2	408559	5	NULL	NULL	0	NULL	mitochondrial - ketoglutarate dehydrogenase complex ( KGDHC )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of the mitochondrial - ketoglutarate dehydrogenase complex ( KGDHC ) in homogenates from autopsy brain declines with AD .
	manualset3
140273	3	408559	5	NULL	NULL	0	NULL	homogenates 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of the mitochondrial - ketoglutarate dehydrogenase complex ( KGDHC ) in homogenates from autopsy brain declines with AD .
	manualset3
140274	4	408559	5	NULL	NULL	0	NULL	autopsy brain 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of the mitochondrial - ketoglutarate dehydrogenase complex ( KGDHC ) in homogenates from autopsy brain declines with AD .
	manualset3
140275	5	408559	5	NULL	NULL	0	NULL	AD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of the mitochondrial - ketoglutarate dehydrogenase complex ( KGDHC ) in homogenates from autopsy brain declines with AD .
	manualset3
140276	1	408560	5	NULL	NULL	0	NULL	activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of the related Sts-2 enzyme is significantly less than that of Sts-1 .
	manualset3
140277	2	408560	5	NULL	NULL	0	NULL	Sts-2 enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of the related Sts-2 enzyme is significantly less than that of Sts-1 .
	manualset3
140278	3	408560	5	NULL	NULL	0	NULL	Sts-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of the related Sts-2 enzyme is significantly less than that of Sts-1 .
	manualset3
140279	1	408561	5	NULL	NULL	0	NULL	activity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of the serratus anterior ( SA ) and trapezius muscles during arm elevation has not been investigated in these patients .
	manualset3
140280	2	408561	5	NULL	NULL	0	NULL	serratus anterior ( SA ) muscles 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of the serratus anterior ( SA ) and trapezius muscles during arm elevation has not been investigated in these patients .
	manualset3
140281	3	408561	5	NULL	NULL	0	NULL	trapezius muscles 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of the serratus anterior ( SA ) and trapezius muscles during arm elevation has not been investigated in these patients .
	manualset3
140282	4	408561	5	NULL	NULL	0	NULL	arm elevation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of the serratus anterior ( SA ) and trapezius muscles during arm elevation has not been investigated in these patients .
	manualset3
140283	5	408561	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of the serratus anterior ( SA ) and trapezius muscles during arm elevation has not been investigated in these patients .
	manualset3
140284	1	408562	5	NULL	NULL	0	NULL	activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of this compound against gram-positive bacteria was higher than those of other quinolones , and its activity against gram-negative and anaerobic bacteria was roughly comparable to those of other quinolones .
	manualset3
140285	2	408562	5	NULL	NULL	0	NULL	compound 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of this compound against gram-positive bacteria was higher than those of other quinolones , and its activity against gram-negative and anaerobic bacteria was roughly comparable to those of other quinolones .
	manualset3
140286	3	408562	5	NULL	NULL	0	NULL	gram-positive bacteria 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of this compound against gram-positive bacteria was higher than those of other quinolones , and its activity against gram-negative and anaerobic bacteria was roughly comparable to those of other quinolones .
	manualset3
140287	4	408562	5	NULL	NULL	0	NULL	quinolones 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of this compound against gram-positive bacteria was higher than those of other quinolones , and its activity against gram-negative and anaerobic bacteria was roughly comparable to those of other quinolones .
	manualset3
140288	5	408562	5	NULL	NULL	0	NULL	activity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of this compound against gram-positive bacteria was higher than those of other quinolones , and its activity against gram-negative and anaerobic bacteria was roughly comparable to those of other quinolones .
	manualset3
140289	6	408562	5	NULL	NULL	0	NULL	gram-negative bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of this compound against gram-positive bacteria was higher than those of other quinolones , and its activity against gram-negative and anaerobic bacteria was roughly comparable to those of other quinolones .
	manualset3
140290	7	408562	5	NULL	NULL	0	NULL	anaerobic bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of this compound against gram-positive bacteria was higher than those of other quinolones , and its activity against gram-negative and anaerobic bacteria was roughly comparable to those of other quinolones .
	manualset3
140291	8	408562	5	NULL	NULL	0	NULL	quinolones 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of this compound against gram-positive bacteria was higher than those of other quinolones , and its activity against gram-negative and anaerobic bacteria was roughly comparable to those of other quinolones .
	manualset3
140292	1	408563	5	NULL	NULL	0	NULL	retrospective analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A retrospective analysis was performed comparing cervical isolation rates , endometrial maturation patterns and laparoscopic findings in 64 patients with SFE and in a control group of 70 unselected patients with no histologic evidence of SFE at endometrial biopsy .
	manualset3
140293	2	408563	5	NULL	NULL	0	NULL	cervical isolation rates 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A retrospective analysis was performed comparing cervical isolation rates , endometrial maturation patterns and laparoscopic findings in 64 patients with SFE and in a control group of 70 unselected patients with no histologic evidence of SFE at endometrial biopsy .
	manualset3
140294	3	408563	5	NULL	NULL	0	NULL	endometrial maturation patterns 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A retrospective analysis was performed comparing cervical isolation rates , endometrial maturation patterns and laparoscopic findings in 64 patients with SFE and in a control group of 70 unselected patients with no histologic evidence of SFE at endometrial biopsy .
	manualset3
140295	4	408563	5	NULL	NULL	0	NULL	laparoscopic findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A retrospective analysis was performed comparing cervical isolation rates , endometrial maturation patterns and laparoscopic findings in 64 patients with SFE and in a control group of 70 unselected patients with no histologic evidence of SFE at endometrial biopsy .
	manualset3
140296	5	408563	5	NULL	NULL	0	NULL	64 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A retrospective analysis was performed comparing cervical isolation rates , endometrial maturation patterns and laparoscopic findings in 64 patients with SFE and in a control group of 70 unselected patients with no histologic evidence of SFE at endometrial biopsy .
	manualset3
140297	6	408563	5	NULL	NULL	0	NULL	SFE 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A retrospective analysis was performed comparing cervical isolation rates , endometrial maturation patterns and laparoscopic findings in 64 patients with SFE and in a control group of 70 unselected patients with no histologic evidence of SFE at endometrial biopsy .
	manualset3
140298	7	408563	5	NULL	NULL	0	NULL	control group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A retrospective analysis was performed comparing cervical isolation rates , endometrial maturation patterns and laparoscopic findings in 64 patients with SFE and in a control group of 70 unselected patients with no histologic evidence of SFE at endometrial biopsy .
	manualset3
140299	8	408563	5	NULL	NULL	0	NULL	 70 unselected patients	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A retrospective analysis was performed comparing cervical isolation rates , endometrial maturation patterns and laparoscopic findings in 64 patients with SFE and in a control group of 70 unselected patients with no histologic evidence of SFE at endometrial biopsy .
	manualset3
140300	9	408563	5	NULL	NULL	0	NULL	histologic evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A retrospective analysis was performed comparing cervical isolation rates , endometrial maturation patterns and laparoscopic findings in 64 patients with SFE and in a control group of 70 unselected patients with no histologic evidence of SFE at endometrial biopsy .
	manualset3
140301	10	408563	5	NULL	NULL	0	NULL	SFE 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A retrospective analysis was performed comparing cervical isolation rates , endometrial maturation patterns and laparoscopic findings in 64 patients with SFE and in a control group of 70 unselected patients with no histologic evidence of SFE at endometrial biopsy .
	manualset3
140302	11	408563	5	NULL	NULL	0	NULL	endometrial biopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A retrospective analysis was performed comparing cervical isolation rates , endometrial maturation patterns and laparoscopic findings in 64 patients with SFE and in a control group of 70 unselected patients with no histologic evidence of SFE at endometrial biopsy .
	manualset3
140303	1	408564	5	NULL	NULL	0	NULL	actual extraction ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The actual extraction ratio was 0.64 + / - 0.04 ( x + / - S.D. , N = 3 ) , which indicated that the rabbit lung was capable of removing a large percentage of circulating benzo ( a ) pyrene 4 , 5-oxide in a single pass through the organ .
	manualset3
140304	2	408564	5	NULL	NULL	0	NULL	0.64 + / - 0.04 ( x + / - S.D. , N = 3 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The actual extraction ratio was 0.64 + / - 0.04 ( x + / - S.D. , N = 3 ) , which indicated that the rabbit lung was capable of removing a large percentage of circulating benzo ( a ) pyrene 4 , 5-oxide in a single pass through the organ .
	manualset3
140305	3	408564	5	NULL	NULL	0	NULL	rabbit lung 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The actual extraction ratio was 0.64 + / - 0.04 ( x + / - S.D. , N = 3 ) , which indicated that the rabbit lung was capable of removing a large percentage of circulating benzo ( a ) pyrene 4 , 5-oxide in a single pass through the organ .
	manualset3
140306	4	408564	5	NULL	NULL	0	NULL	percentage 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The actual extraction ratio was 0.64 + / - 0.04 ( x + / - S.D. , N = 3 ) , which indicated that the rabbit lung was capable of removing a large percentage of circulating benzo ( a ) pyrene 4 , 5-oxide in a single pass through the organ .
	manualset3
140307	5	408564	5	NULL	NULL	0	NULL	benzo ( a ) pyrene 4 , 5-oxide	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The actual extraction ratio was 0.64 + / - 0.04 ( x + / - S.D. , N = 3 ) , which indicated that the rabbit lung was capable of removing a large percentage of circulating benzo ( a ) pyrene 4 , 5-oxide in a single pass through the organ .
	manualset3
140308	6	408564	5	NULL	NULL	0	NULL	organ 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The actual extraction ratio was 0.64 + / - 0.04 ( x + / - S.D. , N = 3 ) , which indicated that the rabbit lung was capable of removing a large percentage of circulating benzo ( a ) pyrene 4 , 5-oxide in a single pass through the organ .
	manualset3
140309	1	408565	5	NULL	NULL	0	NULL	actual limit	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The actual limit of reproductive cell life would therefore not likely be reached in a normal life-span .
	manualset3
140310	2	408565	5	NULL	NULL	0	NULL	reproductive cell life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The actual limit of reproductive cell life would therefore not likely be reached in a normal life-span .
	manualset3
140311	3	408565	5	NULL	NULL	0	NULL	normal life-span 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The actual limit of reproductive cell life would therefore not likely be reached in a normal life-span .
	manualset3
140312	1	408566	5	NULL	NULL	0	NULL	acute insulin secretory response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The acute insulin secretory response to 10 mM theophylline was maintained after culture .
	manualset3
140313	2	408566	5	NULL	NULL	0	NULL	10 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The acute insulin secretory response to 10 mM theophylline was maintained after culture .
	manualset3
140314	3	408566	5	NULL	NULL	0	NULL	theophylline 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The acute insulin secretory response to 10 mM theophylline was maintained after culture .
	manualset3
140315	4	408566	5	NULL	NULL	0	NULL	culture 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The acute insulin secretory response to 10 mM theophylline was maintained after culture .
	manualset3
140316	1	408567	5	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of FBS attenuates this effect .
	manualset3
140317	2	408567	5	NULL	NULL	0	NULL	FBS 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of FBS attenuates this effect .
	manualset3
140318	3	408567	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of FBS attenuates this effect .
	manualset3
140319	1	408568	5	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of GnRH failed to alter testosterone ( T ) or progesterone secretion or germinal vesicle breakdown over a wide dose range of gonadotropin .
	manualset3
140320	2	408568	5	NULL	NULL	0	NULL	GnRH 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of GnRH failed to alter testosterone ( T ) or progesterone secretion or germinal vesicle breakdown over a wide dose range of gonadotropin .
	manualset3
140321	3	408568	5	NULL	NULL	0	NULL	testosterone ( T ) secretion 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of GnRH failed to alter testosterone ( T ) or progesterone secretion or germinal vesicle breakdown over a wide dose range of gonadotropin .
	manualset3
140322	4	408568	5	NULL	NULL	0	NULL	progesterone secretion 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of GnRH failed to alter testosterone ( T ) or progesterone secretion or germinal vesicle breakdown over a wide dose range of gonadotropin .
	manualset3
140323	5	408568	5	NULL	NULL	0	NULL	germinal vesicle breakdown	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of GnRH failed to alter testosterone ( T ) or progesterone secretion or germinal vesicle breakdown over a wide dose range of gonadotropin .
	manualset3
140324	6	408568	5	NULL	NULL	0	NULL	wide dose range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of GnRH failed to alter testosterone ( T ) or progesterone secretion or germinal vesicle breakdown over a wide dose range of gonadotropin .
	manualset3
140325	7	408568	5	NULL	NULL	0	NULL	gonadotropin 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of GnRH failed to alter testosterone ( T ) or progesterone secretion or germinal vesicle breakdown over a wide dose range of gonadotropin .
	manualset3
140326	1	408569	5	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of atropine reverses these responses completely .
	manualset3
140327	2	408569	5	NULL	NULL	0	NULL	atropine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of atropine reverses these responses completely .
	manualset3
140328	3	408569	5	NULL	NULL	0	NULL	responses 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of atropine reverses these responses completely .
	manualset3
140329	1	408570	5	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of clopidogrel to aspirin for patients undergoing percutaneous coronary intervention ( PCI ) had significantly reduced cardiovascular events .
	manualset3
140330	2	408570	5	NULL	NULL	0	NULL	clopidogrel 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of clopidogrel to aspirin for patients undergoing percutaneous coronary intervention ( PCI ) had significantly reduced cardiovascular events .
	manualset3
140331	3	408570	5	NULL	NULL	0	NULL	aspirin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of clopidogrel to aspirin for patients undergoing percutaneous coronary intervention ( PCI ) had significantly reduced cardiovascular events .
	manualset3
140332	4	408570	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of clopidogrel to aspirin for patients undergoing percutaneous coronary intervention ( PCI ) had significantly reduced cardiovascular events .
	manualset3
140333	5	408570	5	NULL	NULL	0	NULL	percutaneous coronary intervention ( PCI )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of clopidogrel to aspirin for patients undergoing percutaneous coronary intervention ( PCI ) had significantly reduced cardiovascular events .
	manualset3
140334	6	408570	5	NULL	NULL	0	NULL	cardiovascular events 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of clopidogrel to aspirin for patients undergoing percutaneous coronary intervention ( PCI ) had significantly reduced cardiovascular events .
	manualset3
140335	1	408571	5	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of curcumin or celecoxib to the IFN-alpha-pretreated A549 cells altered the IFN-alpha sensitivity of cell growth inhibition .
	manualset3
140336	2	408571	5	NULL	NULL	0	NULL	curcumin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of curcumin or celecoxib to the IFN-alpha-pretreated A549 cells altered the IFN-alpha sensitivity of cell growth inhibition .
	manualset3
140337	3	408571	5	NULL	NULL	0	NULL	celecoxib 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of curcumin or celecoxib to the IFN-alpha-pretreated A549 cells altered the IFN-alpha sensitivity of cell growth inhibition .
	manualset3
140338	4	408571	5	NULL	NULL	0	NULL	 IFN-alpha-pretreated A549 cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of curcumin or celecoxib to the IFN-alpha-pretreated A549 cells altered the IFN-alpha sensitivity of cell growth inhibition .
	manualset3
140339	5	408571	5	NULL	NULL	0	NULL	IFN-alpha sensitivity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of curcumin or celecoxib to the IFN-alpha-pretreated A549 cells altered the IFN-alpha sensitivity of cell growth inhibition .
	manualset3
140340	6	408571	5	NULL	NULL	0	NULL	cell growth inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of curcumin or celecoxib to the IFN-alpha-pretreated A549 cells altered the IFN-alpha sensitivity of cell growth inhibition .
	manualset3
140341	1	408572	5	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of plasminogen and streptokinase to rabbit serum results in appearance of chemotactic activity which is relatively heat-labile and dialyzable .
	manualset3
140342	2	408572	5	NULL	NULL	0	NULL	plasminogen 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of plasminogen and streptokinase to rabbit serum results in appearance of chemotactic activity which is relatively heat-labile and dialyzable .
	manualset3
140343	3	408572	5	NULL	NULL	0	NULL	streptokinase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of plasminogen and streptokinase to rabbit serum results in appearance of chemotactic activity which is relatively heat-labile and dialyzable .
	manualset3
140344	4	408572	5	NULL	NULL	0	NULL	rabbit serum 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of plasminogen and streptokinase to rabbit serum results in appearance of chemotactic activity which is relatively heat-labile and dialyzable .
	manualset3
140345	5	408572	5	NULL	NULL	0	NULL	appearance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of plasminogen and streptokinase to rabbit serum results in appearance of chemotactic activity which is relatively heat-labile and dialyzable .
	manualset3
140346	6	408572	5	NULL	NULL	0	NULL	chemotactic activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of plasminogen and streptokinase to rabbit serum results in appearance of chemotactic activity which is relatively heat-labile and dialyzable .
	manualset3
140347	1	408573	5	NULL	NULL	0	NULL	additive effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The additive effect of acetazolamide and ouabain on pancreatic secretion in vitro .
	manualset3
140348	2	408573	5	NULL	NULL	0	NULL	acetazolamide 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The additive effect of acetazolamide and ouabain on pancreatic secretion in vitro .
	manualset3
140349	3	408573	5	NULL	NULL	0	NULL	ouabain 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The additive effect of acetazolamide and ouabain on pancreatic secretion in vitro .
	manualset3
140350	4	408573	5	NULL	NULL	0	NULL	pancreatic secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The additive effect of acetazolamide and ouabain on pancreatic secretion in vitro .
	manualset3
140351	1	408574	5	NULL	NULL	0	NULL	additive genetic variance	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The additive genetic variance reflects a population 's intrinsic potential to respond to selection .
	manualset3
140352	2	408574	5	NULL	NULL	0	NULL	intrinsic potential	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The additive genetic variance reflects a population 's intrinsic potential to respond to selection .
	manualset3
140353	3	408574	5	NULL	NULL	NULL	NULL	respond to selection 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The additive genetic variance reflects a population 's intrinsic potential to respond to selection .
	manualset3
142892	4	408574	5	NULL	NULL	0	NULL	population 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The additive genetic variance reflects a population 's intrinsic potential to respond to selection .
	manualset3
140354	1	408575	5	NULL	NULL	0	NULL	adenosine analog 5 , 6-dichloro-1-beta-D-ribofuranosylbenzimidazole ( DRB )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The adenosine analog 5 , 6-dichloro-1-beta-D-ribofuranosylbenzimidazole ( DRB ) is a specific inhibitor for RNA polymerase II transcription in vivo and in vitro ( Tamm + Sehgal ( 1978 ) Adv .
	manualset3
140355	2	408575	5	NULL	NULL	0	NULL	specific inhibitor	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The adenosine analog 5 , 6-dichloro-1-beta-D-ribofuranosylbenzimidazole ( DRB ) is a specific inhibitor for RNA polymerase II transcription in vivo and in vitro ( Tamm + Sehgal ( 1978 ) Adv .
	manualset3
140356	3	408575	5	NULL	NULL	0	NULL	RNA polymerase II transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The adenosine analog 5 , 6-dichloro-1-beta-D-ribofuranosylbenzimidazole ( DRB ) is a specific inhibitor for RNA polymerase II transcription in vivo and in vitro ( Tamm + Sehgal ( 1978 ) Adv .
	manualset3
140357	4	408575	5	NULL	NULL	0	NULL	Tamm + Sehgal (1978) Adv.	Citation												NULL		0	NULL	NULL	NULL	NULL	NULL	The adenosine analog 5 , 6-dichloro-1-beta-D-ribofuranosylbenzimidazole ( DRB ) is a specific inhibitor for RNA polymerase II transcription in vivo and in vitro ( Tamm + Sehgal ( 1978 ) Adv .
	manualset3
140358	1	408576	5	NULL	NULL	0	NULL	adhesive proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The adhesive proteins compete reciprocally for binding to GPIIb/IIIa , and the complex binds to different domains of them , thus creating multiple interactions with the ligands .
	manualset3
140359	2	408576	5	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The adhesive proteins compete reciprocally for binding to GPIIb/IIIa , and the complex binds to different domains of them , thus creating multiple interactions with the ligands .
	manualset3
140360	3	408576	5	NULL	NULL	0	NULL	GPIIb/IIIa	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The adhesive proteins compete reciprocally for binding to GPIIb/IIIa , and the complex binds to different domains of them , thus creating multiple interactions with the ligands .
	manualset3
140361	4	408576	5	NULL	NULL	0	NULL	complex 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The adhesive proteins compete reciprocally for binding to GPIIb/IIIa , and the complex binds to different domains of them , thus creating multiple interactions with the ligands .
	manualset3
140362	5	408576	5	NULL	NULL	0	NULL	domains 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The adhesive proteins compete reciprocally for binding to GPIIb/IIIa , and the complex binds to different domains of them , thus creating multiple interactions with the ligands .
	manualset3
140363	6	408576	5	NULL	NULL	0	NULL	interactions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The adhesive proteins compete reciprocally for binding to GPIIb/IIIa , and the complex binds to different domains of them , thus creating multiple interactions with the ligands .
	manualset3
140364	7	408576	5	NULL	NULL	0	NULL	ligands 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The adhesive proteins compete reciprocally for binding to GPIIb/IIIa , and the complex binds to different domains of them , thus creating multiple interactions with the ligands .
	manualset3
140365	1	408577	5	NULL	NULL	0	NULL	ratio 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The adjusted odds ratio as an estimate of relative risk for VTE was 2.3 ( 0.8-7 .0 ; 95 % confidence interval ) .
	manualset3
140366	2	408577	5	NULL	NULL	NULL	NULL	relative risk	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The adjusted odds ratio as an estimate of relative risk for VTE was 2.3 ( 0.8-7 .0 ; 95 % confidence interval ) .
	manualset3
140367	3	408577	5	NULL	NULL	0	NULL	VTE	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The adjusted odds ratio as an estimate of relative risk for VTE was 2.3 ( 0.8-7 .0 ; 95 % confidence interval ) .
	manualset3
140368	4	408577	5	NULL	NULL	0	NULL	2.3 ( 0.8-7 .0 ; 95 % confidence interval )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The adjusted odds ratio as an estimate of relative risk for VTE was 2.3 ( 0.8-7 .0 ; 95 % confidence interval ) .
	manualset3
140369	1	408578	5	NULL	NULL	0	NULL	administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The administration of GnRH stimulated GH release in 12 out of the 16 diabetics and in 8 out of the 18 depressed patients , but not in the normal controls .
	manualset3
140370	2	408578	5	NULL	NULL	0	NULL	GnRH 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The administration of GnRH stimulated GH release in 12 out of the 16 diabetics and in 8 out of the 18 depressed patients , but not in the normal controls .
	manualset3
140371	3	408578	5	NULL	NULL	0	NULL	GH release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The administration of GnRH stimulated GH release in 12 out of the 16 diabetics and in 8 out of the 18 depressed patients , but not in the normal controls .
	manualset3
140372	4	408578	5	NULL	NULL	0	NULL	12 out of the 16 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The administration of GnRH stimulated GH release in 12 out of the 16 diabetics and in 8 out of the 18 depressed patients , but not in the normal controls .
	manualset3
140373	5	408578	5	NULL	NULL	0	NULL	diabetics 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The administration of GnRH stimulated GH release in 12 out of the 16 diabetics and in 8 out of the 18 depressed patients , but not in the normal controls .
	manualset3
140374	6	408578	5	NULL	NULL	0	NULL	8 out of the 18	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The administration of GnRH stimulated GH release in 12 out of the 16 diabetics and in 8 out of the 18 depressed patients , but not in the normal controls .
	manualset3
140375	7	408578	5	NULL	NULL	0	NULL	depressed patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The administration of GnRH stimulated GH release in 12 out of the 16 diabetics and in 8 out of the 18 depressed patients , but not in the normal controls .
	manualset3
140376	8	408578	5	NULL	NULL	0	NULL	normal controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The administration of GnRH stimulated GH release in 12 out of the 16 diabetics and in 8 out of the 18 depressed patients , but not in the normal controls .
	manualset3
140377	1	408579	5	NULL	NULL	0	NULL	administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The administration of IL-1 alpha accelerated the recovery from this suppression .
	manualset3
140378	2	408579	5	NULL	NULL	0	NULL	 IL-1 alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The administration of IL-1 alpha accelerated the recovery from this suppression .
	manualset3
140379	3	408579	5	NULL	NULL	0	NULL	recovery 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The administration of IL-1 alpha accelerated the recovery from this suppression .
	manualset3
140380	4	408579	5	NULL	NULL	0	NULL	suppression 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The administration of IL-1 alpha accelerated the recovery from this suppression .
	manualset3
140381	1	408580	5	NULL	NULL	0	NULL	administration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The administration of alcohol led husbands , but not wives , to increase their problem-solving attempts .
	manualset3
140382	2	408580	5	NULL	NULL	0	NULL	alcohol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The administration of alcohol led husbands , but not wives , to increase their problem-solving attempts .
	manualset3
140383	3	408580	5	NULL	NULL	0	NULL	husbands 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The administration of alcohol led husbands , but not wives , to increase their problem-solving attempts .
	manualset3
140384	4	408580	5	NULL	NULL	0	NULL	wives 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The administration of alcohol led husbands , but not wives , to increase their problem-solving attempts .
	manualset3
140385	5	408580	5	NULL	NULL	0	NULL	problem-solving attempts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The administration of alcohol led husbands , but not wives , to increase their problem-solving attempts .
	manualset3
140386	1	408581	5	NULL	NULL	0	NULL	administration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The administration of an institution has the primary responsibility for the visible implementation of risk and safety management .
	manualset3
140387	2	408581	5	NULL	NULL	0	NULL	institution 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The administration of an institution has the primary responsibility for the visible implementation of risk and safety management .
	manualset3
140388	3	408581	5	NULL	NULL	0	NULL	responsibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The administration of an institution has the primary responsibility for the visible implementation of risk and safety management .
	manualset3
140389	4	408581	5	NULL	NULL	0	NULL	visible implementation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The administration of an institution has the primary responsibility for the visible implementation of risk and safety management .
	manualset3
140390	5	408581	5	NULL	NULL	0	NULL	risk 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The administration of an institution has the primary responsibility for the visible implementation of risk and safety management .
	manualset3
140391	6	408581	5	NULL	NULL	0	NULL	safety management 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The administration of an institution has the primary responsibility for the visible implementation of risk and safety management .
	manualset3
140392	1	408582	5	NULL	NULL	0	NULL	adoption 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The adoption of the Ag Guide by the AAALAC Board of Trustees as a primary standard signifies its importance in the AAALAC accreditation process .
	manualset3
140393	2	408582	5	NULL	NULL	0	NULL	Ag Guide	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The adoption of the Ag Guide by the AAALAC Board of Trustees as a primary standard signifies its importance in the AAALAC accreditation process .
	manualset3
140394	3	408582	5	NULL	NULL	0	NULL	AAALAC Board of Trustees	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The adoption of the Ag Guide by the AAALAC Board of Trustees as a primary standard signifies its importance in the AAALAC accreditation process .
	manualset3
140395	4	408582	5	NULL	NULL	0	NULL	primary standard	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The adoption of the Ag Guide by the AAALAC Board of Trustees as a primary standard signifies its importance in the AAALAC accreditation process .
	manualset3
140396	5	408582	5	NULL	NULL	0	NULL	importance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The adoption of the Ag Guide by the AAALAC Board of Trustees as a primary standard signifies its importance in the AAALAC accreditation process .
	manualset3
140398	6	408582	5	NULL	NULL	0	NULL	AAALAC accreditation process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The adoption of the Ag Guide by the AAALAC Board of Trustees as a primary standard signifies its importance in the AAALAC accreditation process .
	manualset3
140399	1	408583	5	NULL	NULL	0	NULL	adult SMN model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The adult SMN model provides a good opportunity to investigate the reexpression of LNGFR after peripheral nerve injury , and more generally , the unknown role and regulation of LNGFR .
	manualset3
140400	2	408583	5	NULL	NULL	0	NULL	opportunity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The adult SMN model provides a good opportunity to investigate the reexpression of LNGFR after peripheral nerve injury , and more generally , the unknown role and regulation of LNGFR .
	manualset3
140401	3	408583	5	NULL	NULL	0	NULL	reexpression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The adult SMN model provides a good opportunity to investigate the reexpression of LNGFR after peripheral nerve injury , and more generally , the unknown role and regulation of LNGFR .
	manualset3
140402	4	408583	5	NULL	NULL	0	NULL	LNGFR 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The adult SMN model provides a good opportunity to investigate the reexpression of LNGFR after peripheral nerve injury , and more generally , the unknown role and regulation of LNGFR .
	manualset3
140403	5	408583	5	NULL	NULL	0	NULL	peripheral nerve injury	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The adult SMN model provides a good opportunity to investigate the reexpression of LNGFR after peripheral nerve injury , and more generally , the unknown role and regulation of LNGFR .
	manualset3
140404	6	408583	5	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The adult SMN model provides a good opportunity to investigate the reexpression of LNGFR after peripheral nerve injury , and more generally , the unknown role and regulation of LNGFR .
	manualset3
140405	7	408583	5	NULL	NULL	NULL	NULL	regulation 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The adult SMN model provides a good opportunity to investigate the reexpression of LNGFR after peripheral nerve injury , and more generally , the unknown role and regulation of LNGFR .
	manualset3
140406	8	408583	5	NULL	NULL	0	NULL	LNGFR 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The adult SMN model provides a good opportunity to investigate the reexpression of LNGFR after peripheral nerve injury , and more generally , the unknown role and regulation of LNGFR .
	manualset3
140407	1	408584	5	NULL	NULL	0	NULL	advantage 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The advantage of this simple , fast , and accurate procedure is that no hardware change or upgrade is needed .
	manualset3
140408	2	408584	5	NULL	NULL	0	NULL	simple , fast , and accurate procedure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The advantage of this simple , fast , and accurate procedure is that no hardware change or upgrade is needed .
	manualset3
140409	3	408584	5	NULL	NULL	0	NULL	hardware change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The advantage of this simple , fast , and accurate procedure is that no hardware change or upgrade is needed .
	manualset3
140410	4	408584	5	NULL	NULL	0	NULL	upgrade 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The advantage of this simple , fast , and accurate procedure is that no hardware change or upgrade is needed .
	manualset3
140411	1	408585	5	NULL	NULL	0	NULL	retrospective study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A retrospective study demonstrated that the costs of HLA-B 1502 screening were less than those of SJS treatment .
	manualset3
140412	2	408585	5	NULL	NULL	0	NULL	costs 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A retrospective study demonstrated that the costs of HLA-B 1502 screening were less than those of SJS treatment .
	manualset3
140413	3	408585	5	NULL	NULL	0	NULL	 HLA-B 1502 screening 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A retrospective study demonstrated that the costs of HLA-B 1502 screening were less than those of SJS treatment .
	manualset3
140414	4	408585	5	NULL	NULL	0	NULL	SJS treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A retrospective study demonstrated that the costs of HLA-B 1502 screening were less than those of SJS treatment .
	manualset3
140415	1	408586	5	NULL	NULL	0	NULL	advantages 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The advantages of dabigatran are its more predictable response , obviating coagulation monitoring and possible lower frequency of bleedings .
	manualset3
140416	2	408586	5	NULL	NULL	0	NULL	dabigatran 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The advantages of dabigatran are its more predictable response , obviating coagulation monitoring and possible lower frequency of bleedings .
	manualset3
140417	3	408586	5	NULL	NULL	0	NULL	predictable response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The advantages of dabigatran are its more predictable response , obviating coagulation monitoring and possible lower frequency of bleedings .
	manualset3
140418	4	408586	5	NULL	NULL	0	NULL	coagulation monitoring	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The advantages of dabigatran are its more predictable response , obviating coagulation monitoring and possible lower frequency of bleedings .
	manualset3
140419	5	408586	5	NULL	NULL	0	NULL	lower frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The advantages of dabigatran are its more predictable response , obviating coagulation monitoring and possible lower frequency of bleedings .
	manualset3
140420	6	408586	5	NULL	NULL	0	NULL	bleedings 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The advantages of dabigatran are its more predictable response , obviating coagulation monitoring and possible lower frequency of bleedings .
	manualset3
140421	1	408587	5	NULL	NULL	0	NULL	advantages 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The advantages of the technique are smaller sample sizes ( only 5 ml . )
	manualset3
140422	2	408587	5	NULL	NULL	0	NULL	technique 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The advantages of the technique are smaller sample sizes ( only 5 ml . )
	manualset3
140423	3	408587	5	NULL	NULL	0	NULL	smaller sample sizes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The advantages of the technique are smaller sample sizes ( only 5 ml . )
	manualset3
140424	4	408587	5	NULL	NULL	0	NULL	5 ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The advantages of the technique are smaller sample sizes ( only 5 ml . )
	manualset3
140425	1	408588	5	NULL	NULL	0	NULL	adverse impact 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The adverse impact on recovery of posttraumatic stress disorder ( PTSD ) in mild traumatic brain injury ( TBI ) has been demonstrated in returned veterans .
	manualset3
140426	2	408588	5	NULL	NULL	0	NULL	recovery 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The adverse impact on recovery of posttraumatic stress disorder ( PTSD ) in mild traumatic brain injury ( TBI ) has been demonstrated in returned veterans .
	manualset3
140427	3	408588	5	NULL	NULL	0	NULL	posttraumatic stress disorder ( PTSD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The adverse impact on recovery of posttraumatic stress disorder ( PTSD ) in mild traumatic brain injury ( TBI ) has been demonstrated in returned veterans .
	manualset3
140428	4	408588	5	NULL	NULL	0	NULL	mild traumatic brain injury ( TBI )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The adverse impact on recovery of posttraumatic stress disorder ( PTSD ) in mild traumatic brain injury ( TBI ) has been demonstrated in returned veterans .
	manualset3
140429	5	408588	5	NULL	NULL	0	NULL	veterans 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The adverse impact on recovery of posttraumatic stress disorder ( PTSD ) in mild traumatic brain injury ( TBI ) has been demonstrated in returned veterans .
	manualset3
140430	1	408589	5	NULL	NULL	0	NULL	aetiology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aetiology and physiological characteristics differ from those of chronic renal failure ( CRF ) and both conditions should be approached differently .
	manualset3
140431	2	408589	5	NULL	NULL	0	NULL	physiological characteristics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aetiology and physiological characteristics differ from those of chronic renal failure ( CRF ) and both conditions should be approached differently .
	manualset3
140432	3	408589	5	NULL	NULL	0	NULL	chronic renal failure ( CRF ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The aetiology and physiological characteristics differ from those of chronic renal failure ( CRF ) and both conditions should be approached differently .
	manualset3
140433	4	408589	5	NULL	NULL	0	NULL	conditions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aetiology and physiological characteristics differ from those of chronic renal failure ( CRF ) and both conditions should be approached differently .
	manualset3
140434	1	408590	5	NULL	NULL	NULL	NULL	subject 	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The affected subject has an android build , with more facial and body hair than in previously described affected adults .
	manualset3
140435	2	408590	5	NULL	NULL	0	NULL	android build	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The affected subject has an android build , with more facial and body hair than in previously described affected adults .
	manualset3
140436	3	408590	5	NULL	NULL	0	NULL	facial hair	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The affected subject has an android build , with more facial and body hair than in previously described affected adults .
	manualset3
140437	4	408590	5	NULL	NULL	0	NULL	body hair	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The affected subject has an android build , with more facial and body hair than in previously described affected adults .
	manualset3
140438	5	408590	5	NULL	NULL	0	NULL	adults 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The affected subject has an android build , with more facial and body hair than in previously described affected adults .
	manualset3
140439	1	408591	5	NULL	NULL	0	NULL	affinity 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The affinity and enantioselectivity have been determined for designed propranolol derivatives as ligands for Cel7A by capillary electrophoresis ( CE ) at pH 7.0 .
	manualset3
140440	2	408591	5	NULL	NULL	0	NULL	enantioselectivity 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The affinity and enantioselectivity have been determined for designed propranolol derivatives as ligands for Cel7A by capillary electrophoresis ( CE ) at pH 7.0 .
	manualset3
140441	3	408591	5	NULL	NULL	0	NULL	propranolol derivatives 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The affinity and enantioselectivity have been determined for designed propranolol derivatives as ligands for Cel7A by capillary electrophoresis ( CE ) at pH 7.0 .
	manualset3
140442	4	408591	5	NULL	NULL	0	NULL	ligands 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The affinity and enantioselectivity have been determined for designed propranolol derivatives as ligands for Cel7A by capillary electrophoresis ( CE ) at pH 7.0 .
	manualset3
140443	5	408591	5	NULL	NULL	0	NULL	Cel7A 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The affinity and enantioselectivity have been determined for designed propranolol derivatives as ligands for Cel7A by capillary electrophoresis ( CE ) at pH 7.0 .
	manualset3
140444	6	408591	5	NULL	NULL	0	NULL	capillary electrophoresis ( CE )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The affinity and enantioselectivity have been determined for designed propranolol derivatives as ligands for Cel7A by capillary electrophoresis ( CE ) at pH 7.0 .
	manualset3
140445	7	408591	5	NULL	NULL	0	NULL	pH 7.0	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The affinity and enantioselectivity have been determined for designed propranolol derivatives as ligands for Cel7A by capillary electrophoresis ( CE ) at pH 7.0 .
	manualset3
140446	1	408592	5	NULL	NULL	0	NULL	affinity 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The affinity of ( ( 3 ) H ) benzylpenicillin for penicillin-binding protein ( PBP ) 3A was reduced in 25 clinical isolates of beta-lactamase-negative ampicillin ( AMP ) - resistant ( BLNAR ) Haemophilus influenzae for which the AMP MIC was ) or = 1.0 microg/ml .
	manualset3
140447	2	408592	5	NULL	NULL	0	NULL	 ( ( 3 ) H ) benzylpenicillin	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The affinity of ( ( 3 ) H ) benzylpenicillin for penicillin-binding protein ( PBP ) 3A was reduced in 25 clinical isolates of beta-lactamase-negative ampicillin ( AMP ) - resistant ( BLNAR ) Haemophilus influenzae for which the AMP MIC was ) or = 1.0 microg/ml .
	manualset3
140448	3	408592	5	NULL	NULL	0	NULL	penicillin-binding protein ( PBP ) 3A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The affinity of ( ( 3 ) H ) benzylpenicillin for penicillin-binding protein ( PBP ) 3A was reduced in 25 clinical isolates of beta-lactamase-negative ampicillin ( AMP ) - resistant ( BLNAR ) Haemophilus influenzae for which the AMP MIC was ) or = 1.0 microg/ml .
	manualset3
140449	4	408592	5	NULL	NULL	0	NULL	25 clinical isolates 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The affinity of ( ( 3 ) H ) benzylpenicillin for penicillin-binding protein ( PBP ) 3A was reduced in 25 clinical isolates of beta-lactamase-negative ampicillin ( AMP ) - resistant ( BLNAR ) Haemophilus influenzae for which the AMP MIC was ) or = 1.0 microg/ml .
	manualset3
140450	5	408592	5	NULL	NULL	0	NULL	beta-lactamase-negative ampicillin ( AMP ) - resistant ( BLNAR ) Haemophilus influenzae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The affinity of ( ( 3 ) H ) benzylpenicillin for penicillin-binding protein ( PBP ) 3A was reduced in 25 clinical isolates of beta-lactamase-negative ampicillin ( AMP ) - resistant ( BLNAR ) Haemophilus influenzae for which the AMP MIC was ) or = 1.0 microg/ml .
	manualset3
140451	6	408592	5	NULL	NULL	0	NULL	AMP MIC	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The affinity of ( ( 3 ) H ) benzylpenicillin for penicillin-binding protein ( PBP ) 3A was reduced in 25 clinical isolates of beta-lactamase-negative ampicillin ( AMP ) - resistant ( BLNAR ) Haemophilus influenzae for which the AMP MIC was ) or = 1.0 microg/ml .
	manualset3
140452	7	408592	5	NULL	NULL	0	NULL	= 1.0 microg/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The affinity of ( ( 3 ) H ) benzylpenicillin for penicillin-binding protein ( PBP ) 3A was reduced in 25 clinical isolates of beta-lactamase-negative ampicillin ( AMP ) - resistant ( BLNAR ) Haemophilus influenzae for which the AMP MIC was ) or = 1.0 microg/ml .
	manualset3
140453	1	408593	5	NULL	NULL	0	NULL	affinity 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The affinity of Hb Zurich for carbon monoxide is approximately 65 times that of normal hemoglobin .
	manualset3
140454	2	408593	5	NULL	NULL	NULL	NULL	Hb Zurich	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The affinity of Hb Zurich for carbon monoxide is approximately 65 times that of normal hemoglobin .
	manualset3
140455	3	408593	5	NULL	NULL	0	NULL	carbon monoxide	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The affinity of Hb Zurich for carbon monoxide is approximately 65 times that of normal hemoglobin .
	manualset3
140456	4	408593	5	NULL	NULL	0	NULL	65 times	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The affinity of Hb Zurich for carbon monoxide is approximately 65 times that of normal hemoglobin .
	manualset3
140457	5	408593	5	NULL	NULL	0	NULL	hemoglobin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The affinity of Hb Zurich for carbon monoxide is approximately 65 times that of normal hemoglobin .
	manualset3
140458	1	408594	5	NULL	NULL	NULL	NULL	affinity 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The affinity of a series of 2 ' , 3 ' - and 5-modified thymidine analogs for Mycobacterium tuberculosis thymidine monophosphate kinase ( TMPKmt ) was evaluated .
	manualset3
140459	2	408594	5	NULL	NULL	0	NULL	 2 ' , 3 ' - and 5-modified thymidine analogs	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The affinity of a series of 2 ' , 3 ' - and 5-modified thymidine analogs for Mycobacterium tuberculosis thymidine monophosphate kinase ( TMPKmt ) was evaluated .
	manualset3
140460	3	408594	5	NULL	NULL	0	NULL	Mycobacterium tuberculosis thymidine monophosphate kinase ( TMPKmt ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The affinity of a series of 2 ' , 3 ' - and 5-modified thymidine analogs for Mycobacterium tuberculosis thymidine monophosphate kinase ( TMPKmt ) was evaluated .
	manualset3
140461	1	408595	5	NULL	NULL	0	NULL	affinity 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The affinity of albumin for zinc added to serum from pregnant women was less than that of albumin from non-pregnant women .
	manualset3
140462	2	408595	5	NULL	NULL	0	NULL	albumin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The affinity of albumin for zinc added to serum from pregnant women was less than that of albumin from non-pregnant women .
	manualset3
140463	3	408595	5	NULL	NULL	0	NULL	zinc 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The affinity of albumin for zinc added to serum from pregnant women was less than that of albumin from non-pregnant women .
	manualset3
140464	4	408595	5	NULL	NULL	0	NULL	serum 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The affinity of albumin for zinc added to serum from pregnant women was less than that of albumin from non-pregnant women .
	manualset3
140465	5	408595	5	NULL	NULL	0	NULL	pregnant women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The affinity of albumin for zinc added to serum from pregnant women was less than that of albumin from non-pregnant women .
	manualset3
140466	6	408595	5	NULL	NULL	0	NULL	albumin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The affinity of albumin for zinc added to serum from pregnant women was less than that of albumin from non-pregnant women .
	manualset3
140467	7	408595	5	NULL	NULL	0	NULL	non-pregnant women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The affinity of albumin for zinc added to serum from pregnant women was less than that of albumin from non-pregnant women .
	manualset3
140468	1	408596	5	NULL	NULL	0	NULL	age - and sex-matched control group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The age - and sex-matched control group of 50 patients had exclusion of coronary artery disease by angiography , and normal left ventricular ( ejection fraction 55 % ) and valvular function .
	manualset3
140469	2	408596	5	NULL	NULL	0	NULL	 50 patients	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The age - and sex-matched control group of 50 patients had exclusion of coronary artery disease by angiography , and normal left ventricular ( ejection fraction 55 % ) and valvular function .
	manualset3
140470	3	408596	5	NULL	NULL	0	NULL	exclusion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The age - and sex-matched control group of 50 patients had exclusion of coronary artery disease by angiography , and normal left ventricular ( ejection fraction 55 % ) and valvular function .
	manualset3
140471	4	408596	5	NULL	NULL	0	NULL	coronary artery disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The age - and sex-matched control group of 50 patients had exclusion of coronary artery disease by angiography , and normal left ventricular ( ejection fraction 55 % ) and valvular function .
	manualset3
140472	5	408596	5	NULL	NULL	0	NULL	angiography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The age - and sex-matched control group of 50 patients had exclusion of coronary artery disease by angiography , and normal left ventricular ( ejection fraction 55 % ) and valvular function .
	manualset3
140473	6	408596	5	NULL	NULL	0	NULL	normal left ventricular function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The age - and sex-matched control group of 50 patients had exclusion of coronary artery disease by angiography , and normal left ventricular ( ejection fraction 55 % ) and valvular function .
	manualset3
140474	7	408596	5	NULL	NULL	0	NULL	ejection fraction 55 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The age - and sex-matched control group of 50 patients had exclusion of coronary artery disease by angiography , and normal left ventricular ( ejection fraction 55 % ) and valvular function .
	manualset3
140475	8	408596	5	NULL	NULL	0	NULL	valvular function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The age - and sex-matched control group of 50 patients had exclusion of coronary artery disease by angiography , and normal left ventricular ( ejection fraction 55 % ) and valvular function .
	manualset3
140476	1	408597	5	NULL	NULL	0	NULL	age	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The age and physical state of the patient , the accuracy of reduction , and the security of fixation had the greatest influence on union .
	manualset3
140477	2	408597	5	NULL	NULL	0	NULL	physical state	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The age and physical state of the patient , the accuracy of reduction , and the security of fixation had the greatest influence on union .
	manualset3
140478	3	408597	5	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The age and physical state of the patient , the accuracy of reduction , and the security of fixation had the greatest influence on union .
	manualset3
140479	4	408597	5	NULL	NULL	NULL	NULL	 accuracy of reduction	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The age and physical state of the patient , the accuracy of reduction , and the security of fixation had the greatest influence on union .
	manualset3
140480	5	408597	5	NULL	NULL	NULL	NULL	security of fixation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The age and physical state of the patient , the accuracy of reduction , and the security of fixation had the greatest influence on union .
	manualset3
140481	6	408597	5	NULL	NULL	0	NULL	influence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The age and physical state of the patient , the accuracy of reduction , and the security of fixation had the greatest influence on union .
	manualset3
140482	7	408597	5	NULL	NULL	0	NULL	union 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The age and physical state of the patient , the accuracy of reduction , and the security of fixation had the greatest influence on union .
	manualset3
140483	1	408598	5	NULL	NULL	0	NULL	agent 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The agent is superior to the conventional combination of 50 % analgin ( 2 ml ) and 1 % dimedrolum ( 1 ml ) in its efficiency and duration of action .
	manualset3
140484	2	408598	5	NULL	NULL	0	NULL	conventional combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The agent is superior to the conventional combination of 50 % analgin ( 2 ml ) and 1 % dimedrolum ( 1 ml ) in its efficiency and duration of action .
	manualset3
140485	3	408598	5	NULL	NULL	0	NULL	 50 % analgin ( 2 ml ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The agent is superior to the conventional combination of 50 % analgin ( 2 ml ) and 1 % dimedrolum ( 1 ml ) in its efficiency and duration of action .
	manualset3
140486	4	408598	5	NULL	NULL	0	NULL	1 % dimedrolum ( 1 ml ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The agent is superior to the conventional combination of 50 % analgin ( 2 ml ) and 1 % dimedrolum ( 1 ml ) in its efficiency and duration of action .
	manualset3
140487	5	408598	5	NULL	NULL	0	NULL	efficiency 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The agent is superior to the conventional combination of 50 % analgin ( 2 ml ) and 1 % dimedrolum ( 1 ml ) in its efficiency and duration of action .
	manualset3
140488	6	408598	5	NULL	NULL	0	NULL	duration of action 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The agent is superior to the conventional combination of 50 % analgin ( 2 ml ) and 1 % dimedrolum ( 1 ml ) in its efficiency and duration of action .
	manualset3
140489	1	408599	5	NULL	NULL	0	NULL	aggregation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aggregation of polyglutamine containing protein sequences is implicated in a family of familial neurodegenerative diseases , the expanded CAG repeat diseases .
	manualset3
140490	2	408599	5	NULL	NULL	0	NULL	polyglutamine containing protein sequences	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The aggregation of polyglutamine containing protein sequences is implicated in a family of familial neurodegenerative diseases , the expanded CAG repeat diseases .
	manualset3
140491	3	408599	5	NULL	NULL	0	NULL	family of familial neurodegenerative diseases 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The aggregation of polyglutamine containing protein sequences is implicated in a family of familial neurodegenerative diseases , the expanded CAG repeat diseases .
	manualset3
140492	4	408599	5	NULL	NULL	0	NULL	CAG repeat diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The aggregation of polyglutamine containing protein sequences is implicated in a family of familial neurodegenerative diseases , the expanded CAG repeat diseases .
	manualset3
140493	1	408600	5	NULL	NULL	0	NULL	aging pattern	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aging pattern is observed in population cohorts from the age of 15 years and onward .
	manualset3
140494	2	408600	5	NULL	NULL	0	NULL	population cohorts	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aging pattern is observed in population cohorts from the age of 15 years and onward .
	manualset3
140495	3	408600	5	NULL	NULL	0	NULL	age 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The aging pattern is observed in population cohorts from the age of 15 years and onward .
	manualset3
140496	4	408600	5	NULL	NULL	0	NULL	15 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The aging pattern is observed in population cohorts from the age of 15 years and onward .
	manualset3
140497	1	408601	5	NULL	NULL	0	NULL	retrospective study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A retrospective study of 40 cases with HCC in Israel revealed irregular ( macronodular ) cirrhosis in 37 of 40 cases ( 92.5 % ) .
	manualset3
140498	2	408601	5	NULL	NULL	0	NULL	 40 cases	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A retrospective study of 40 cases with HCC in Israel revealed irregular ( macronodular ) cirrhosis in 37 of 40 cases ( 92.5 % ) .
	manualset3
140499	3	408601	5	NULL	NULL	0	NULL	HCC 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A retrospective study of 40 cases with HCC in Israel revealed irregular ( macronodular ) cirrhosis in 37 of 40 cases ( 92.5 % ) .
	manualset3
140500	4	408601	5	NULL	NULL	0	NULL	Israel 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A retrospective study of 40 cases with HCC in Israel revealed irregular ( macronodular ) cirrhosis in 37 of 40 cases ( 92.5 % ) .
	manualset3
140501	5	408601	5	NULL	NULL	0	NULL	irregular ( macronodular ) cirrhosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A retrospective study of 40 cases with HCC in Israel revealed irregular ( macronodular ) cirrhosis in 37 of 40 cases ( 92.5 % ) .
	manualset3
140502	6	408601	5	NULL	NULL	0	NULL	37 of 40 cases ( 92.5 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A retrospective study of 40 cases with HCC in Israel revealed irregular ( macronodular ) cirrhosis in 37 of 40 cases ( 92.5 % ) .
	manualset3
140503	1	408602	5	NULL	NULL	0	NULL	agonist binding site 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The agonist binding site of the nicotinic acetylcholine receptor has a loop-based structure , and is formed by residues located remotely to each other in terms of primary structure .
	manualset3
140504	2	408602	5	NULL	NULL	0	NULL	nicotinic acetylcholine receptor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The agonist binding site of the nicotinic acetylcholine receptor has a loop-based structure , and is formed by residues located remotely to each other in terms of primary structure .
	manualset3
140505	3	408602	5	NULL	NULL	0	NULL	loop-based structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The agonist binding site of the nicotinic acetylcholine receptor has a loop-based structure , and is formed by residues located remotely to each other in terms of primary structure .
	manualset3
140506	4	408602	5	NULL	NULL	0	NULL	residues 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The agonist binding site of the nicotinic acetylcholine receptor has a loop-based structure , and is formed by residues located remotely to each other in terms of primary structure .
	manualset3
140507	5	408602	5	NULL	NULL	0	NULL	primary structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The agonist binding site of the nicotinic acetylcholine receptor has a loop-based structure , and is formed by residues located remotely to each other in terms of primary structure .
	manualset3
140508	1	408603	5	NULL	NULL	0	NULL	agreement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The agreement between the measured and predicted breakthrough of sulfate and copper was good .
	manualset3
140509	2	408603	5	NULL	NULL	0	NULL	measured breakthrough 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The agreement between the measured and predicted breakthrough of sulfate and copper was good .
	manualset3
140510	3	408603	5	NULL	NULL	0	NULL	predicted breakthrough 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The agreement between the measured and predicted breakthrough of sulfate and copper was good .
	manualset3
140511	4	408603	5	NULL	NULL	0	NULL	sulfate 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The agreement between the measured and predicted breakthrough of sulfate and copper was good .
	manualset3
140512	5	408603	5	NULL	NULL	0	NULL	copper 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The agreement between the measured and predicted breakthrough of sulfate and copper was good .
	manualset3
140513	1	408604	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim is to demonstrate that such a dialectic tool and method of representation may assist the ergonomist to frame the essence of a work activity in practical terms , swiftly and in a manner that preserves its multifaceted unity .
	manualset3
140514	2	408604	5	NULL	NULL	0	NULL	dialectic tool	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim is to demonstrate that such a dialectic tool and method of representation may assist the ergonomist to frame the essence of a work activity in practical terms , swiftly and in a manner that preserves its multifaceted unity .
	manualset3
140515	3	408604	5	NULL	NULL	NULL	NULL	method of representation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The aim is to demonstrate that such a dialectic tool and method of representation may assist the ergonomist to frame the essence of a work activity in practical terms , swiftly and in a manner that preserves its multifaceted unity .
	manualset3
140516	4	408604	5	NULL	NULL	0	NULL	ergonomist 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim is to demonstrate that such a dialectic tool and method of representation may assist the ergonomist to frame the essence of a work activity in practical terms , swiftly and in a manner that preserves its multifaceted unity .
	manualset3
140517	5	408604	5	NULL	NULL	0	NULL	essence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim is to demonstrate that such a dialectic tool and method of representation may assist the ergonomist to frame the essence of a work activity in practical terms , swiftly and in a manner that preserves its multifaceted unity .
	manualset3
140518	6	408604	5	NULL	NULL	0	NULL	work activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim is to demonstrate that such a dialectic tool and method of representation may assist the ergonomist to frame the essence of a work activity in practical terms , swiftly and in a manner that preserves its multifaceted unity .
	manualset3
140519	7	408604	5	NULL	NULL	0	NULL	practical terms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim is to demonstrate that such a dialectic tool and method of representation may assist the ergonomist to frame the essence of a work activity in practical terms , swiftly and in a manner that preserves its multifaceted unity .
	manualset3
140520	8	408604	5	NULL	NULL	0	NULL	manner 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim is to demonstrate that such a dialectic tool and method of representation may assist the ergonomist to frame the essence of a work activity in practical terms , swiftly and in a manner that preserves its multifaceted unity .
	manualset3
140521	9	408604	5	NULL	NULL	0	NULL	multifaceted unity	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim is to demonstrate that such a dialectic tool and method of representation may assist the ergonomist to frame the essence of a work activity in practical terms , swiftly and in a manner that preserves its multifaceted unity .
	manualset3
140522	1	408605	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim is to reproduce a main lobe profile as close as possible to the desired one through the synthesis of the array-weighting window .
	manualset3
140523	2	408605	5	NULL	NULL	0	NULL	main lobe profile 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim is to reproduce a main lobe profile as close as possible to the desired one through the synthesis of the array-weighting window .
	manualset3
140524	3	408605	5	NULL	NULL	0	NULL	synthesis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim is to reproduce a main lobe profile as close as possible to the desired one through the synthesis of the array-weighting window .
	manualset3
140525	4	408605	5	NULL	NULL	0	NULL	array-weighting window	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim is to reproduce a main lobe profile as close as possible to the desired one through the synthesis of the array-weighting window .
	manualset3
140526	1	408606	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of chemotherapy is to achieve a good clinical response rather than CCR of liver metastasis .
	manualset3
140527	2	408606	5	NULL	NULL	0	NULL	chemotherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of chemotherapy is to achieve a good clinical response rather than CCR of liver metastasis .
	manualset3
140528	3	408606	5	NULL	NULL	0	NULL	good clinical response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of chemotherapy is to achieve a good clinical response rather than CCR of liver metastasis .
	manualset3
140529	4	408606	5	NULL	NULL	0	NULL	CCR 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of chemotherapy is to achieve a good clinical response rather than CCR of liver metastasis .
	manualset3
140530	5	408606	5	NULL	NULL	0	NULL	liver metastasis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of chemotherapy is to achieve a good clinical response rather than CCR of liver metastasis .
	manualset3
140531	1	408607	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the clinical study was to monitor and analyze possible causes of chronic venous insufficiency ( CVI ) in a randomised sample of patients with diagnosed CVI .
	manualset3
140532	2	408607	5	NULL	NULL	0	NULL	clinical study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the clinical study was to monitor and analyze possible causes of chronic venous insufficiency ( CVI ) in a randomised sample of patients with diagnosed CVI .
	manualset3
140533	3	408607	5	NULL	NULL	0	NULL	causes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the clinical study was to monitor and analyze possible causes of chronic venous insufficiency ( CVI ) in a randomised sample of patients with diagnosed CVI .
	manualset3
140534	4	408607	5	NULL	NULL	0	NULL	chronic venous insufficiency ( CVI ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the clinical study was to monitor and analyze possible causes of chronic venous insufficiency ( CVI ) in a randomised sample of patients with diagnosed CVI .
	manualset3
140535	5	408607	5	NULL	NULL	0	NULL	randomised sample 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the clinical study was to monitor and analyze possible causes of chronic venous insufficiency ( CVI ) in a randomised sample of patients with diagnosed CVI .
	manualset3
140536	6	408607	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the clinical study was to monitor and analyze possible causes of chronic venous insufficiency ( CVI ) in a randomised sample of patients with diagnosed CVI .
	manualset3
140537	7	408607	5	NULL	NULL	0	NULL	CVI 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the clinical study was to monitor and analyze possible causes of chronic venous insufficiency ( CVI ) in a randomised sample of patients with diagnosed CVI .
	manualset3
140538	1	408608	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the current investigation was to study the effect of cryo-procedures on canine sperm P4 receptor ( s ) .
	manualset3
140539	2	408608	5	NULL	NULL	0	NULL	investigation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the current investigation was to study the effect of cryo-procedures on canine sperm P4 receptor ( s ) .
	manualset3
140541	4	408608	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the current investigation was to study the effect of cryo-procedures on canine sperm P4 receptor ( s ) .
	manualset3
140542	5	408608	5	NULL	NULL	NULL	NULL	cryo-procedures	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The aim of the current investigation was to study the effect of cryo-procedures on canine sperm P4 receptor ( s ) .
	manualset3
140543	6	408608	5	NULL	NULL	0	NULL	canine sperm P4 receptor ( s )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the current investigation was to study the effect of cryo-procedures on canine sperm P4 receptor ( s ) .
	manualset3
140544	1	408609	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present 2-year follow-up study among young managers ( N = 433 ) was to investigate the intraindividual developmental patterns of burnout and work engagement as well as their interconnections .
	manualset3
140545	2	408609	5	NULL	NULL	0	NULL	 2-year follow-up study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present 2-year follow-up study among young managers ( N = 433 ) was to investigate the intraindividual developmental patterns of burnout and work engagement as well as their interconnections .
	manualset3
140546	3	408609	5	NULL	NULL	0	NULL	young managers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present 2-year follow-up study among young managers ( N = 433 ) was to investigate the intraindividual developmental patterns of burnout and work engagement as well as their interconnections .
	manualset3
140547	4	408609	5	NULL	NULL	0	NULL	N = 433	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present 2-year follow-up study among young managers ( N = 433 ) was to investigate the intraindividual developmental patterns of burnout and work engagement as well as their interconnections .
	manualset3
140548	5	408609	5	NULL	NULL	0	NULL	intraindividual developmental patterns	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present 2-year follow-up study among young managers ( N = 433 ) was to investigate the intraindividual developmental patterns of burnout and work engagement as well as their interconnections .
	manualset3
140549	6	408609	5	NULL	NULL	0	NULL	burnout 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present 2-year follow-up study among young managers ( N = 433 ) was to investigate the intraindividual developmental patterns of burnout and work engagement as well as their interconnections .
	manualset3
140550	7	408609	5	NULL	NULL	0	NULL	work engagement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present 2-year follow-up study among young managers ( N = 433 ) was to investigate the intraindividual developmental patterns of burnout and work engagement as well as their interconnections .
	manualset3
140551	8	408609	5	NULL	NULL	0	NULL	interconnections 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present 2-year follow-up study among young managers ( N = 433 ) was to investigate the intraindividual developmental patterns of burnout and work engagement as well as their interconnections .
	manualset3
140552	1	408610	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to characterize further the putative novel R , mediating these P effects in the murine Leydig tumor cell line , mLTC-1 .
	manualset3
140553	2	408610	5	NULL	NULL	0	NULL	present study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to characterize further the putative novel R , mediating these P effects in the murine Leydig tumor cell line , mLTC-1 .
	manualset3
142893	3	408610	5	NULL	NULL	0	NULL	putative novel R	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to characterize further the putative novel R , mediating these P effects in the murine Leydig tumor cell line , mLTC-1 .
	manualset3
142894	4	408610	5	NULL	NULL	0	NULL	P effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to characterize further the putative novel R , mediating these P effects in the murine Leydig tumor cell line , mLTC-1 .
	manualset3
142895	5	408610	5	NULL	NULL	NULL	NULL	murine Leydig tumor cell line , mLTC-1	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to characterize further the putative novel R , mediating these P effects in the murine Leydig tumor cell line , mLTC-1 .
	manualset3
140554	1	408611	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to determine the dimensions of the mandible during the fetal period , the relationship between the growth rates of the angle of the mandible and the dimensions of the mandible .
	manualset3
140555	2	408611	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to determine the dimensions of the mandible during the fetal period , the relationship between the growth rates of the angle of the mandible and the dimensions of the mandible .
	manualset3
140556	3	408611	5	NULL	NULL	0	NULL	dimensions 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to determine the dimensions of the mandible during the fetal period , the relationship between the growth rates of the angle of the mandible and the dimensions of the mandible .
	manualset3
140557	4	408611	5	NULL	NULL	0	NULL	mandible 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to determine the dimensions of the mandible during the fetal period , the relationship between the growth rates of the angle of the mandible and the dimensions of the mandible .
	manualset3
140558	5	408611	5	NULL	NULL	0	NULL	fetal period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to determine the dimensions of the mandible during the fetal period , the relationship between the growth rates of the angle of the mandible and the dimensions of the mandible .
	manualset3
140559	6	408611	5	NULL	NULL	0	NULL	relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to determine the dimensions of the mandible during the fetal period , the relationship between the growth rates of the angle of the mandible and the dimensions of the mandible .
	manualset3
140560	7	408611	5	NULL	NULL	0	NULL	growth rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to determine the dimensions of the mandible during the fetal period , the relationship between the growth rates of the angle of the mandible and the dimensions of the mandible .
	manualset3
140561	8	408611	5	NULL	NULL	0	NULL	angle 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to determine the dimensions of the mandible during the fetal period , the relationship between the growth rates of the angle of the mandible and the dimensions of the mandible .
	manualset3
140562	9	408611	5	NULL	NULL	0	NULL	mandible 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to determine the dimensions of the mandible during the fetal period , the relationship between the growth rates of the angle of the mandible and the dimensions of the mandible .
	manualset3
140563	10	408611	5	NULL	NULL	0	NULL	dimensions 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to determine the dimensions of the mandible during the fetal period , the relationship between the growth rates of the angle of the mandible and the dimensions of the mandible .
	manualset3
140564	11	408611	5	NULL	NULL	0	NULL	mandible 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to determine the dimensions of the mandible during the fetal period , the relationship between the growth rates of the angle of the mandible and the dimensions of the mandible .
	manualset3
140565	1	408612	5	NULL	NULL	0	NULL	retrospective study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A retrospective study was performed on 169 beef and dairy calves aged from 1 to 7 days old submitted to the Diagnostic Laboratories at INTA Balcarce , Argentina .
	manualset3
140566	2	408612	5	NULL	NULL	0	NULL	169 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A retrospective study was performed on 169 beef and dairy calves aged from 1 to 7 days old submitted to the Diagnostic Laboratories at INTA Balcarce , Argentina .
	manualset3
140567	3	408612	5	NULL	NULL	0	NULL	beef 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A retrospective study was performed on 169 beef and dairy calves aged from 1 to 7 days old submitted to the Diagnostic Laboratories at INTA Balcarce , Argentina .
	manualset3
140568	4	408612	5	NULL	NULL	0	NULL	dairy calves 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A retrospective study was performed on 169 beef and dairy calves aged from 1 to 7 days old submitted to the Diagnostic Laboratories at INTA Balcarce , Argentina .
	manualset3
140569	5	408612	5	NULL	NULL	0	NULL	 1 to 7 days old 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A retrospective study was performed on 169 beef and dairy calves aged from 1 to 7 days old submitted to the Diagnostic Laboratories at INTA Balcarce , Argentina .
	manualset3
140570	6	408612	5	NULL	NULL	0	NULL	Diagnostic Laboratories	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A retrospective study was performed on 169 beef and dairy calves aged from 1 to 7 days old submitted to the Diagnostic Laboratories at INTA Balcarce , Argentina .
	manualset3
140571	7	408612	5	NULL	NULL	0	NULL	INTA Balcarce , Argentina 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A retrospective study was performed on 169 beef and dairy calves aged from 1 to 7 days old submitted to the Diagnostic Laboratories at INTA Balcarce , Argentina .
	manualset3
140572	1	408613	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to examine fetal brain activation to sound , using fMRI at the beginning of the third trimester of pregnancy .
	manualset3
140573	2	408613	5	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to examine fetal brain activation to sound , using fMRI at the beginning of the third trimester of pregnancy .
	manualset3
140574	3	408613	5	NULL	NULL	0	NULL	fetal brain activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to examine fetal brain activation to sound , using fMRI at the beginning of the third trimester of pregnancy .
	manualset3
140575	4	408613	5	NULL	NULL	0	NULL	sound 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to examine fetal brain activation to sound , using fMRI at the beginning of the third trimester of pregnancy .
	manualset3
140576	5	408613	5	NULL	NULL	0	NULL	fMRI 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to examine fetal brain activation to sound , using fMRI at the beginning of the third trimester of pregnancy .
	manualset3
140577	6	408613	5	NULL	NULL	0	NULL	third trimester	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to examine fetal brain activation to sound , using fMRI at the beginning of the third trimester of pregnancy .
	manualset3
140578	7	408613	5	NULL	NULL	0	NULL	pregnancy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to examine fetal brain activation to sound , using fMRI at the beginning of the third trimester of pregnancy .
	manualset3
140579	1	408614	5	NULL	NULL	0	NULL	aim	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to measure the incorporation of infused 15N in blood fractions , urine , digesta , faeces and in the exocrine pancreatic and biliary secretions , in order to estimate the endogenous part of nitrogen in the ileal digesta and in the faeces of pigs fed a casein diet and to calculate the total endogenous nitrogen secretion as well as its recycling in the digestive tract .
	manualset3
140580	2	408614	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to measure the incorporation of infused 15N in blood fractions , urine , digesta , faeces and in the exocrine pancreatic and biliary secretions , in order to estimate the endogenous part of nitrogen in the ileal digesta and in the faeces of pigs fed a casein diet and to calculate the total endogenous nitrogen secretion as well as its recycling in the digestive tract .
	manualset3
140581	3	408614	5	NULL	NULL	0	NULL	incorporation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to measure the incorporation of infused 15N in blood fractions , urine , digesta , faeces and in the exocrine pancreatic and biliary secretions , in order to estimate the endogenous part of nitrogen in the ileal digesta and in the faeces of pigs fed a casein diet and to calculate the total endogenous nitrogen secretion as well as its recycling in the digestive tract .
	manualset3
140582	4	408614	5	NULL	NULL	0	NULL	15N	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to measure the incorporation of infused 15N in blood fractions , urine , digesta , faeces and in the exocrine pancreatic and biliary secretions , in order to estimate the endogenous part of nitrogen in the ileal digesta and in the faeces of pigs fed a casein diet and to calculate the total endogenous nitrogen secretion as well as its recycling in the digestive tract .
	manualset3
140583	5	408614	5	NULL	NULL	0	NULL	 blood fractions 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to measure the incorporation of infused 15N in blood fractions , urine , digesta , faeces and in the exocrine pancreatic and biliary secretions , in order to estimate the endogenous part of nitrogen in the ileal digesta and in the faeces of pigs fed a casein diet and to calculate the total endogenous nitrogen secretion as well as its recycling in the digestive tract .
	manualset3
140584	6	408614	5	NULL	NULL	0	NULL	urine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to measure the incorporation of infused 15N in blood fractions , urine , digesta , faeces and in the exocrine pancreatic and biliary secretions , in order to estimate the endogenous part of nitrogen in the ileal digesta and in the faeces of pigs fed a casein diet and to calculate the total endogenous nitrogen secretion as well as its recycling in the digestive tract .
	manualset3
140585	7	408614	5	NULL	NULL	0	NULL	digesta 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to measure the incorporation of infused 15N in blood fractions , urine , digesta , faeces and in the exocrine pancreatic and biliary secretions , in order to estimate the endogenous part of nitrogen in the ileal digesta and in the faeces of pigs fed a casein diet and to calculate the total endogenous nitrogen secretion as well as its recycling in the digestive tract .
	manualset3
140586	8	408614	5	NULL	NULL	0	NULL	faeces 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to measure the incorporation of infused 15N in blood fractions , urine , digesta , faeces and in the exocrine pancreatic and biliary secretions , in order to estimate the endogenous part of nitrogen in the ileal digesta and in the faeces of pigs fed a casein diet and to calculate the total endogenous nitrogen secretion as well as its recycling in the digestive tract .
	manualset3
140587	9	408614	5	NULL	NULL	0	NULL	exocrine pancreatic secretions 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to measure the incorporation of infused 15N in blood fractions , urine , digesta , faeces and in the exocrine pancreatic and biliary secretions , in order to estimate the endogenous part of nitrogen in the ileal digesta and in the faeces of pigs fed a casein diet and to calculate the total endogenous nitrogen secretion as well as its recycling in the digestive tract .
	manualset3
140588	10	408614	5	NULL	NULL	0	NULL	biliary secretions 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to measure the incorporation of infused 15N in blood fractions , urine , digesta , faeces and in the exocrine pancreatic and biliary secretions , in order to estimate the endogenous part of nitrogen in the ileal digesta and in the faeces of pigs fed a casein diet and to calculate the total endogenous nitrogen secretion as well as its recycling in the digestive tract .
	manualset3
140589	11	408614	5	NULL	NULL	0	NULL	endogenous part	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to measure the incorporation of infused 15N in blood fractions , urine , digesta , faeces and in the exocrine pancreatic and biliary secretions , in order to estimate the endogenous part of nitrogen in the ileal digesta and in the faeces of pigs fed a casein diet and to calculate the total endogenous nitrogen secretion as well as its recycling in the digestive tract .
	manualset3
140590	12	408614	5	NULL	NULL	0	NULL	nitrogen 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to measure the incorporation of infused 15N in blood fractions , urine , digesta , faeces and in the exocrine pancreatic and biliary secretions , in order to estimate the endogenous part of nitrogen in the ileal digesta and in the faeces of pigs fed a casein diet and to calculate the total endogenous nitrogen secretion as well as its recycling in the digestive tract .
	manualset3
140591	13	408614	5	NULL	NULL	0	NULL	ileal digesta	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to measure the incorporation of infused 15N in blood fractions , urine , digesta , faeces and in the exocrine pancreatic and biliary secretions , in order to estimate the endogenous part of nitrogen in the ileal digesta and in the faeces of pigs fed a casein diet and to calculate the total endogenous nitrogen secretion as well as its recycling in the digestive tract .
	manualset3
140592	14	408614	5	NULL	NULL	0	NULL	faeces 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to measure the incorporation of infused 15N in blood fractions , urine , digesta , faeces and in the exocrine pancreatic and biliary secretions , in order to estimate the endogenous part of nitrogen in the ileal digesta and in the faeces of pigs fed a casein diet and to calculate the total endogenous nitrogen secretion as well as its recycling in the digestive tract .
	manualset3
140593	15	408614	5	NULL	NULL	0	NULL	pigs 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to measure the incorporation of infused 15N in blood fractions , urine , digesta , faeces and in the exocrine pancreatic and biliary secretions , in order to estimate the endogenous part of nitrogen in the ileal digesta and in the faeces of pigs fed a casein diet and to calculate the total endogenous nitrogen secretion as well as its recycling in the digestive tract .
	manualset3
140594	16	408614	5	NULL	NULL	0	NULL	casein diet 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to measure the incorporation of infused 15N in blood fractions , urine , digesta , faeces and in the exocrine pancreatic and biliary secretions , in order to estimate the endogenous part of nitrogen in the ileal digesta and in the faeces of pigs fed a casein diet and to calculate the total endogenous nitrogen secretion as well as its recycling in the digestive tract .
	manualset3
140595	17	408614	5	NULL	NULL	0	NULL	total endogenous nitrogen secretion 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to measure the incorporation of infused 15N in blood fractions , urine , digesta , faeces and in the exocrine pancreatic and biliary secretions , in order to estimate the endogenous part of nitrogen in the ileal digesta and in the faeces of pigs fed a casein diet and to calculate the total endogenous nitrogen secretion as well as its recycling in the digestive tract .
	manualset3
140596	18	408614	5	NULL	NULL	0	NULL	digestive tract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to measure the incorporation of infused 15N in blood fractions , urine , digesta , faeces and in the exocrine pancreatic and biliary secretions , in order to estimate the endogenous part of nitrogen in the ileal digesta and in the faeces of pigs fed a casein diet and to calculate the total endogenous nitrogen secretion as well as its recycling in the digestive tract .
	manualset3
140597	1	408615	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to test the capacity of protein kinase C ( PKC ) to phosphorylate EBP50 and to regulate its oligomerization .
	manualset3
140598	2	408615	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to test the capacity of protein kinase C ( PKC ) to phosphorylate EBP50 and to regulate its oligomerization .
	manualset3
140599	3	408615	5	NULL	NULL	0	NULL	test 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to test the capacity of protein kinase C ( PKC ) to phosphorylate EBP50 and to regulate its oligomerization .
	manualset3
140600	4	408615	5	NULL	NULL	0	NULL	capacity 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to test the capacity of protein kinase C ( PKC ) to phosphorylate EBP50 and to regulate its oligomerization .
	manualset3
140601	5	408615	5	NULL	NULL	0	NULL	protein kinase C ( PKC ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to test the capacity of protein kinase C ( PKC ) to phosphorylate EBP50 and to regulate its oligomerization .
	manualset3
140602	6	408615	5	NULL	NULL	0	NULL	EBP50 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to test the capacity of protein kinase C ( PKC ) to phosphorylate EBP50 and to regulate its oligomerization .
	manualset3
140603	7	408615	5	NULL	NULL	0	NULL	oligomerization 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present study was to test the capacity of protein kinase C ( PKC ) to phosphorylate EBP50 and to regulate its oligomerization .
	manualset3
140604	1	408616	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to assess the expression of agouti-like protein and neuropeptide Y in pregnant and lactating mice and to compare this with the leptin level and food consumption .
	manualset3
140606	3	408616	5	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to assess the expression of agouti-like protein and neuropeptide Y in pregnant and lactating mice and to compare this with the leptin level and food consumption .
	manualset3
140607	4	408616	5	NULL	NULL	0	NULL	agouti-like protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to assess the expression of agouti-like protein and neuropeptide Y in pregnant and lactating mice and to compare this with the leptin level and food consumption .
	manualset3
140608	5	408616	5	NULL	NULL	0	NULL	neuropeptide Y	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to assess the expression of agouti-like protein and neuropeptide Y in pregnant and lactating mice and to compare this with the leptin level and food consumption .
	manualset3
140610	6	408616	5	NULL	NULL	0	NULL	pregnant mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to assess the expression of agouti-like protein and neuropeptide Y in pregnant and lactating mice and to compare this with the leptin level and food consumption .
	manualset3
140611	7	408616	5	NULL	NULL	0	NULL	lactating mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to assess the expression of agouti-like protein and neuropeptide Y in pregnant and lactating mice and to compare this with the leptin level and food consumption .
	manualset3
140612	8	408616	5	NULL	NULL	0	NULL	leptin level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to assess the expression of agouti-like protein and neuropeptide Y in pregnant and lactating mice and to compare this with the leptin level and food consumption .
	manualset3
140613	9	408616	5	NULL	NULL	0	NULL	food consumption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to assess the expression of agouti-like protein and neuropeptide Y in pregnant and lactating mice and to compare this with the leptin level and food consumption .
	manualset3
140614	1	408617	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to develop a new multiparticulate system , designed for colon-specific delivery of celecoxib for both systemic ( in chronotherapic treatment of arthritis ) and local ( in prophylaxis of colon carcinogenesis ) therapy .
	manualset3
140616	2	408617	5	NULL	NULL	0	NULL	multiparticulate system	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to develop a new multiparticulate system , designed for colon-specific delivery of celecoxib for both systemic ( in chronotherapic treatment of arthritis ) and local ( in prophylaxis of colon carcinogenesis ) therapy .
	manualset3
140617	3	408617	5	NULL	NULL	0	NULL	colon-specific delivery 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to develop a new multiparticulate system , designed for colon-specific delivery of celecoxib for both systemic ( in chronotherapic treatment of arthritis ) and local ( in prophylaxis of colon carcinogenesis ) therapy .
	manualset3
140618	4	408617	5	NULL	NULL	0	NULL	celecoxib 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to develop a new multiparticulate system , designed for colon-specific delivery of celecoxib for both systemic ( in chronotherapic treatment of arthritis ) and local ( in prophylaxis of colon carcinogenesis ) therapy .
	manualset3
140619	5	408617	5	NULL	NULL	0	NULL	systemic therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to develop a new multiparticulate system , designed for colon-specific delivery of celecoxib for both systemic ( in chronotherapic treatment of arthritis ) and local ( in prophylaxis of colon carcinogenesis ) therapy .
	manualset3
140620	6	408617	5	NULL	NULL	0	NULL	chronotherapic treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to develop a new multiparticulate system , designed for colon-specific delivery of celecoxib for both systemic ( in chronotherapic treatment of arthritis ) and local ( in prophylaxis of colon carcinogenesis ) therapy .
	manualset3
140621	7	408617	5	NULL	NULL	0	NULL	arthritis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to develop a new multiparticulate system , designed for colon-specific delivery of celecoxib for both systemic ( in chronotherapic treatment of arthritis ) and local ( in prophylaxis of colon carcinogenesis ) therapy .
	manualset3
140622	8	408617	5	NULL	NULL	0	NULL	local therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to develop a new multiparticulate system , designed for colon-specific delivery of celecoxib for both systemic ( in chronotherapic treatment of arthritis ) and local ( in prophylaxis of colon carcinogenesis ) therapy .
	manualset3
140623	9	408617	5	NULL	NULL	0	NULL	prophylaxis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to develop a new multiparticulate system , designed for colon-specific delivery of celecoxib for both systemic ( in chronotherapic treatment of arthritis ) and local ( in prophylaxis of colon carcinogenesis ) therapy .
	manualset3
140624	10	408617	5	NULL	NULL	0	NULL	colon carcinogenesis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to develop a new multiparticulate system , designed for colon-specific delivery of celecoxib for both systemic ( in chronotherapic treatment of arthritis ) and local ( in prophylaxis of colon carcinogenesis ) therapy .
	manualset3
142896	11	408617	5	NULL	NULL	0	NULL	work 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to develop a new multiparticulate system , designed for colon-specific delivery of celecoxib for both systemic ( in chronotherapic treatment of arthritis ) and local ( in prophylaxis of colon carcinogenesis ) therapy .
	manualset3
140625	1	408618	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to investigate the effect of ageing on DNA alteration events by RAPD ( random amplification of polymorphic DNA ) analysis and to determine whether loss of seed viability might correspond to a controlled programmed cell death ( PCD ) .
	manualset3
140626	2	408618	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to investigate the effect of ageing on DNA alteration events by RAPD ( random amplification of polymorphic DNA ) analysis and to determine whether loss of seed viability might correspond to a controlled programmed cell death ( PCD ) .
	manualset3
140627	3	408618	5	NULL	NULL	0	NULL	ageing 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to investigate the effect of ageing on DNA alteration events by RAPD ( random amplification of polymorphic DNA ) analysis and to determine whether loss of seed viability might correspond to a controlled programmed cell death ( PCD ) .
	manualset3
140628	4	408618	5	NULL	NULL	0	NULL	DNA alteration	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to investigate the effect of ageing on DNA alteration events by RAPD ( random amplification of polymorphic DNA ) analysis and to determine whether loss of seed viability might correspond to a controlled programmed cell death ( PCD ) .
	manualset3
140629	5	408618	5	NULL	NULL	0	NULL	RAPD ( random amplification of polymorphic DNA ) analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to investigate the effect of ageing on DNA alteration events by RAPD ( random amplification of polymorphic DNA ) analysis and to determine whether loss of seed viability might correspond to a controlled programmed cell death ( PCD ) .
	manualset3
140630	6	408618	5	NULL	NULL	0	NULL	loss 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to investigate the effect of ageing on DNA alteration events by RAPD ( random amplification of polymorphic DNA ) analysis and to determine whether loss of seed viability might correspond to a controlled programmed cell death ( PCD ) .
	manualset3
140631	7	408618	5	NULL	NULL	0	NULL	seed viability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to investigate the effect of ageing on DNA alteration events by RAPD ( random amplification of polymorphic DNA ) analysis and to determine whether loss of seed viability might correspond to a controlled programmed cell death ( PCD ) .
	manualset3
140632	8	408618	5	NULL	NULL	0	NULL	programmed cell death ( PCD )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to investigate the effect of ageing on DNA alteration events by RAPD ( random amplification of polymorphic DNA ) analysis and to determine whether loss of seed viability might correspond to a controlled programmed cell death ( PCD ) .
	manualset3
142897	9	408618	5	NULL	NULL	0	NULL	work 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to investigate the effect of ageing on DNA alteration events by RAPD ( random amplification of polymorphic DNA ) analysis and to determine whether loss of seed viability might correspond to a controlled programmed cell death ( PCD ) .
	manualset3
140633	1	408619	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to investigate whether identical results could be obtained when the clinical observation of conscious guinea pigs with symptoms of respiratory distress ( bronchoconstriction ) was compared to an objective measuring technique of this parameter .
	manualset3
140634	2	408619	5	NULL	NULL	0	NULL	identical results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to investigate whether identical results could be obtained when the clinical observation of conscious guinea pigs with symptoms of respiratory distress ( bronchoconstriction ) was compared to an objective measuring technique of this parameter .
	manualset3
140635	3	408619	5	NULL	NULL	0	NULL	clinical observation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to investigate whether identical results could be obtained when the clinical observation of conscious guinea pigs with symptoms of respiratory distress ( bronchoconstriction ) was compared to an objective measuring technique of this parameter .
	manualset3
140636	4	408619	5	NULL	NULL	0	NULL	conscious guinea pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to investigate whether identical results could be obtained when the clinical observation of conscious guinea pigs with symptoms of respiratory distress ( bronchoconstriction ) was compared to an objective measuring technique of this parameter .
	manualset3
140637	5	408619	5	NULL	NULL	0	NULL	symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to investigate whether identical results could be obtained when the clinical observation of conscious guinea pigs with symptoms of respiratory distress ( bronchoconstriction ) was compared to an objective measuring technique of this parameter .
	manualset3
140638	6	408619	5	NULL	NULL	0	NULL	respiratory distress ( bronchoconstriction ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to investigate whether identical results could be obtained when the clinical observation of conscious guinea pigs with symptoms of respiratory distress ( bronchoconstriction ) was compared to an objective measuring technique of this parameter .
	manualset3
140639	7	408619	5	NULL	NULL	0	NULL	objective measuring technique 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to investigate whether identical results could be obtained when the clinical observation of conscious guinea pigs with symptoms of respiratory distress ( bronchoconstriction ) was compared to an objective measuring technique of this parameter .
	manualset3
140640	8	408619	5	NULL	NULL	0	NULL	parameter 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to investigate whether identical results could be obtained when the clinical observation of conscious guinea pigs with symptoms of respiratory distress ( bronchoconstriction ) was compared to an objective measuring technique of this parameter .
	manualset3
142898	9	408619	5	NULL	NULL	0	NULL	work 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the present work was to investigate whether identical results could be obtained when the clinical observation of conscious guinea pigs with symptoms of respiratory distress ( bronchoconstriction ) was compared to an objective measuring technique of this parameter .
	manualset3
140641	1	408620	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study is to determine the causes and frequency of hospitalization in HIV-negative boys and adolescents with hemophilia and evaluate their impact on academic achievement .
	manualset3
140642	2	408620	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study is to determine the causes and frequency of hospitalization in HIV-negative boys and adolescents with hemophilia and evaluate their impact on academic achievement .
	manualset3
140643	3	408620	5	NULL	NULL	0	NULL	causes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study is to determine the causes and frequency of hospitalization in HIV-negative boys and adolescents with hemophilia and evaluate their impact on academic achievement .
	manualset3
140644	4	408620	5	NULL	NULL	0	NULL	frequency 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study is to determine the causes and frequency of hospitalization in HIV-negative boys and adolescents with hemophilia and evaluate their impact on academic achievement .
	manualset3
140645	5	408620	5	NULL	NULL	0	NULL	hospitalization 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study is to determine the causes and frequency of hospitalization in HIV-negative boys and adolescents with hemophilia and evaluate their impact on academic achievement .
	manualset3
140646	6	408620	5	NULL	NULL	0	NULL	HIV-negative boys	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study is to determine the causes and frequency of hospitalization in HIV-negative boys and adolescents with hemophilia and evaluate their impact on academic achievement .
	manualset3
140647	7	408620	5	NULL	NULL	0	NULL	adolescents 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study is to determine the causes and frequency of hospitalization in HIV-negative boys and adolescents with hemophilia and evaluate their impact on academic achievement .
	manualset3
140648	8	408620	5	NULL	NULL	0	NULL	hemophilia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study is to determine the causes and frequency of hospitalization in HIV-negative boys and adolescents with hemophilia and evaluate their impact on academic achievement .
	manualset3
140649	9	408620	5	NULL	NULL	0	NULL	impact 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study is to determine the causes and frequency of hospitalization in HIV-negative boys and adolescents with hemophilia and evaluate their impact on academic achievement .
	manualset3
140650	10	408620	5	NULL	NULL	0	NULL	academic achievement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study is to determine the causes and frequency of hospitalization in HIV-negative boys and adolescents with hemophilia and evaluate their impact on academic achievement .
	manualset3
140651	1	408621	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to assess the possible contribution of adrenergic mechanisms to the thermogenic and circulatory effects of glucose ingestion .
	manualset3
140652	2	408621	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to assess the possible contribution of adrenergic mechanisms to the thermogenic and circulatory effects of glucose ingestion .
	manualset3
140653	3	408621	5	NULL	NULL	0	NULL	contribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to assess the possible contribution of adrenergic mechanisms to the thermogenic and circulatory effects of glucose ingestion .
	manualset3
140654	4	408621	5	NULL	NULL	0	NULL	adrenergic mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to assess the possible contribution of adrenergic mechanisms to the thermogenic and circulatory effects of glucose ingestion .
	manualset3
140655	5	408621	5	NULL	NULL	0	NULL	thermogenic effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to assess the possible contribution of adrenergic mechanisms to the thermogenic and circulatory effects of glucose ingestion .
	manualset3
140656	6	408621	5	NULL	NULL	0	NULL	circulatory effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to assess the possible contribution of adrenergic mechanisms to the thermogenic and circulatory effects of glucose ingestion .
	manualset3
140657	7	408621	5	NULL	NULL	0	NULL	glucose ingestion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to assess the possible contribution of adrenergic mechanisms to the thermogenic and circulatory effects of glucose ingestion .
	manualset3
140658	1	408622	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to compare the influence of different collection methods on the results of 17-hydroxyprogesterone measurement in saliva collected by different ways , using commercially available RIAs developed for plasma .
	manualset3
140659	2	408622	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to compare the influence of different collection methods on the results of 17-hydroxyprogesterone measurement in saliva collected by different ways , using commercially available RIAs developed for plasma .
	manualset3
140660	3	408622	5	NULL	NULL	0	NULL	influence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to compare the influence of different collection methods on the results of 17-hydroxyprogesterone measurement in saliva collected by different ways , using commercially available RIAs developed for plasma .
	manualset3
140661	4	408622	5	NULL	NULL	0	NULL	different collection methods	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to compare the influence of different collection methods on the results of 17-hydroxyprogesterone measurement in saliva collected by different ways , using commercially available RIAs developed for plasma .
	manualset3
140662	5	408622	5	NULL	NULL	0	NULL	17-hydroxyprogesterone measurement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to compare the influence of different collection methods on the results of 17-hydroxyprogesterone measurement in saliva collected by different ways , using commercially available RIAs developed for plasma .
	manualset3
140663	6	408622	5	NULL	NULL	0	NULL	saliva 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to compare the influence of different collection methods on the results of 17-hydroxyprogesterone measurement in saliva collected by different ways , using commercially available RIAs developed for plasma .
	manualset3
140664	7	408622	5	NULL	NULL	0	NULL	commercially available RIAs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to compare the influence of different collection methods on the results of 17-hydroxyprogesterone measurement in saliva collected by different ways , using commercially available RIAs developed for plasma .
	manualset3
140665	8	408622	5	NULL	NULL	0	NULL	plasma	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to compare the influence of different collection methods on the results of 17-hydroxyprogesterone measurement in saliva collected by different ways , using commercially available RIAs developed for plasma .
	manualset3
140666	1	408623	5	NULL	NULL	0	NULL	reversal design 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A reversal design was used in which the medications were introduced and withdrawn , and their effects were assessed on various resident behaviors using behavioral and motor performance assessments .
	manualset3
140667	2	408623	5	NULL	NULL	0	NULL	medications 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A reversal design was used in which the medications were introduced and withdrawn , and their effects were assessed on various resident behaviors using behavioral and motor performance assessments .
	manualset3
140668	3	408623	5	NULL	NULL	0	NULL	effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A reversal design was used in which the medications were introduced and withdrawn , and their effects were assessed on various resident behaviors using behavioral and motor performance assessments .
	manualset3
140669	4	408623	5	NULL	NULL	0	NULL	resident behaviors	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A reversal design was used in which the medications were introduced and withdrawn , and their effects were assessed on various resident behaviors using behavioral and motor performance assessments .
	manualset3
140670	5	408623	5	NULL	NULL	0	NULL	behavioral performance assessments	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A reversal design was used in which the medications were introduced and withdrawn , and their effects were assessed on various resident behaviors using behavioral and motor performance assessments .
	manualset3
140671	6	408623	5	NULL	NULL	0	NULL	motor performance assessments	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A reversal design was used in which the medications were introduced and withdrawn , and their effects were assessed on various resident behaviors using behavioral and motor performance assessments .
	manualset3
140672	1	408624	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to compare the numbers and distribution of mast cells in the nasal mucosa of perennial allergic rhinitis ( PAR ) patients and controls , as demonstrated by different staining methods for light microscopy .
	manualset3
140673	2	408624	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to compare the numbers and distribution of mast cells in the nasal mucosa of perennial allergic rhinitis ( PAR ) patients and controls , as demonstrated by different staining methods for light microscopy .
	manualset3
140674	3	408624	5	NULL	NULL	0	NULL	numbers 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to compare the numbers and distribution of mast cells in the nasal mucosa of perennial allergic rhinitis ( PAR ) patients and controls , as demonstrated by different staining methods for light microscopy .
	manualset3
140675	4	408624	5	NULL	NULL	0	NULL	distribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to compare the numbers and distribution of mast cells in the nasal mucosa of perennial allergic rhinitis ( PAR ) patients and controls , as demonstrated by different staining methods for light microscopy .
	manualset3
140676	5	408624	5	NULL	NULL	0	NULL	mast cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to compare the numbers and distribution of mast cells in the nasal mucosa of perennial allergic rhinitis ( PAR ) patients and controls , as demonstrated by different staining methods for light microscopy .
	manualset3
140677	6	408624	5	NULL	NULL	0	NULL	nasal mucosa	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to compare the numbers and distribution of mast cells in the nasal mucosa of perennial allergic rhinitis ( PAR ) patients and controls , as demonstrated by different staining methods for light microscopy .
	manualset3
140678	7	408624	5	NULL	NULL	0	NULL	perennial allergic rhinitis ( PAR ) patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to compare the numbers and distribution of mast cells in the nasal mucosa of perennial allergic rhinitis ( PAR ) patients and controls , as demonstrated by different staining methods for light microscopy .
	manualset3
140679	8	408624	5	NULL	NULL	0	NULL	controls 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to compare the numbers and distribution of mast cells in the nasal mucosa of perennial allergic rhinitis ( PAR ) patients and controls , as demonstrated by different staining methods for light microscopy .
	manualset3
140680	9	408624	5	NULL	NULL	0	NULL	staining methods	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to compare the numbers and distribution of mast cells in the nasal mucosa of perennial allergic rhinitis ( PAR ) patients and controls , as demonstrated by different staining methods for light microscopy .
	manualset3
140681	10	408624	5	NULL	NULL	0	NULL	light microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to compare the numbers and distribution of mast cells in the nasal mucosa of perennial allergic rhinitis ( PAR ) patients and controls , as demonstrated by different staining methods for light microscopy .
	manualset3
140682	1	408625	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to define the ability of 3-carbamoylpyrroline nitroxyl derivative pirolin ( PL ) to mitigate oxidative damage to blood plasma proteins and lipids induced by DOX-DTX chemotherapy in Sprague-Dawley rats bearing DMBA-induced mammary tumor .
	manualset3
140683	2	408625	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to define the ability of 3-carbamoylpyrroline nitroxyl derivative pirolin ( PL ) to mitigate oxidative damage to blood plasma proteins and lipids induced by DOX-DTX chemotherapy in Sprague-Dawley rats bearing DMBA-induced mammary tumor .
	manualset3
140684	3	408625	5	NULL	NULL	0	NULL	ability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to define the ability of 3-carbamoylpyrroline nitroxyl derivative pirolin ( PL ) to mitigate oxidative damage to blood plasma proteins and lipids induced by DOX-DTX chemotherapy in Sprague-Dawley rats bearing DMBA-induced mammary tumor .
	manualset3
140685	4	408625	5	NULL	NULL	0	NULL	3-carbamoylpyrroline nitroxyl derivative pirolin ( PL ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to define the ability of 3-carbamoylpyrroline nitroxyl derivative pirolin ( PL ) to mitigate oxidative damage to blood plasma proteins and lipids induced by DOX-DTX chemotherapy in Sprague-Dawley rats bearing DMBA-induced mammary tumor .
	manualset3
140686	5	408625	5	NULL	NULL	0	NULL	oxidative damage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to define the ability of 3-carbamoylpyrroline nitroxyl derivative pirolin ( PL ) to mitigate oxidative damage to blood plasma proteins and lipids induced by DOX-DTX chemotherapy in Sprague-Dawley rats bearing DMBA-induced mammary tumor .
	manualset3
140687	6	408625	5	NULL	NULL	0	NULL	blood plasma proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to define the ability of 3-carbamoylpyrroline nitroxyl derivative pirolin ( PL ) to mitigate oxidative damage to blood plasma proteins and lipids induced by DOX-DTX chemotherapy in Sprague-Dawley rats bearing DMBA-induced mammary tumor .
	manualset3
140688	7	408625	5	NULL	NULL	0	NULL	lipids 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to define the ability of 3-carbamoylpyrroline nitroxyl derivative pirolin ( PL ) to mitigate oxidative damage to blood plasma proteins and lipids induced by DOX-DTX chemotherapy in Sprague-Dawley rats bearing DMBA-induced mammary tumor .
	manualset3
140689	8	408625	5	NULL	NULL	0	NULL	DOX-DTX chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to define the ability of 3-carbamoylpyrroline nitroxyl derivative pirolin ( PL ) to mitigate oxidative damage to blood plasma proteins and lipids induced by DOX-DTX chemotherapy in Sprague-Dawley rats bearing DMBA-induced mammary tumor .
	manualset3
140690	9	408625	5	NULL	NULL	0	NULL	Sprague-Dawley rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to define the ability of 3-carbamoylpyrroline nitroxyl derivative pirolin ( PL ) to mitigate oxidative damage to blood plasma proteins and lipids induced by DOX-DTX chemotherapy in Sprague-Dawley rats bearing DMBA-induced mammary tumor .
	manualset3
140691	10	408625	5	NULL	NULL	0	NULL	DMBA-induced mammary tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to define the ability of 3-carbamoylpyrroline nitroxyl derivative pirolin ( PL ) to mitigate oxidative damage to blood plasma proteins and lipids induced by DOX-DTX chemotherapy in Sprague-Dawley rats bearing DMBA-induced mammary tumor .
	manualset3
140692	1	408626	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to determine whether such an operation could lower the migration level of contaminants from a multilayer structure ( containing a recycled layer of PET ) to values below the limits required by regulatory agencies .
	manualset3
140693	2	408626	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to determine whether such an operation could lower the migration level of contaminants from a multilayer structure ( containing a recycled layer of PET ) to values below the limits required by regulatory agencies .
	manualset3
140694	3	408626	5	NULL	NULL	0	NULL	operation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to determine whether such an operation could lower the migration level of contaminants from a multilayer structure ( containing a recycled layer of PET ) to values below the limits required by regulatory agencies .
	manualset3
140695	4	408626	5	NULL	NULL	0	NULL	migration level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to determine whether such an operation could lower the migration level of contaminants from a multilayer structure ( containing a recycled layer of PET ) to values below the limits required by regulatory agencies .
	manualset3
140696	5	408626	5	NULL	NULL	0	NULL	contaminants 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to determine whether such an operation could lower the migration level of contaminants from a multilayer structure ( containing a recycled layer of PET ) to values below the limits required by regulatory agencies .
	manualset3
140697	6	408626	5	NULL	NULL	0	NULL	multilayer structure 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to determine whether such an operation could lower the migration level of contaminants from a multilayer structure ( containing a recycled layer of PET ) to values below the limits required by regulatory agencies .
	manualset3
140698	7	408626	5	NULL	NULL	0	NULL	recycled layer of PET 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to determine whether such an operation could lower the migration level of contaminants from a multilayer structure ( containing a recycled layer of PET ) to values below the limits required by regulatory agencies .
	manualset3
140699	8	408626	5	NULL	NULL	0	NULL	values 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to determine whether such an operation could lower the migration level of contaminants from a multilayer structure ( containing a recycled layer of PET ) to values below the limits required by regulatory agencies .
	manualset3
140700	9	408626	5	NULL	NULL	0	NULL	limits 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to determine whether such an operation could lower the migration level of contaminants from a multilayer structure ( containing a recycled layer of PET ) to values below the limits required by regulatory agencies .
	manualset3
140701	10	408626	5	NULL	NULL	0	NULL	regulatory agencies	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to determine whether such an operation could lower the migration level of contaminants from a multilayer structure ( containing a recycled layer of PET ) to values below the limits required by regulatory agencies .
	manualset3
140702	1	408627	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to evaluate the histological response and dimensional ridge alterations following application of a nanocrystalline hydroxyapatite paste ( NHA ) into fresh extraction sockets in dogs .
	manualset3
140703	2	408627	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to evaluate the histological response and dimensional ridge alterations following application of a nanocrystalline hydroxyapatite paste ( NHA ) into fresh extraction sockets in dogs .
	manualset3
140704	3	408627	5	NULL	NULL	0	NULL	histological response	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to evaluate the histological response and dimensional ridge alterations following application of a nanocrystalline hydroxyapatite paste ( NHA ) into fresh extraction sockets in dogs .
	manualset3
140705	4	408627	5	NULL	NULL	0	NULL	dimensional ridge alterations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to evaluate the histological response and dimensional ridge alterations following application of a nanocrystalline hydroxyapatite paste ( NHA ) into fresh extraction sockets in dogs .
	manualset3
140706	5	408627	5	NULL	NULL	0	NULL	application 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to evaluate the histological response and dimensional ridge alterations following application of a nanocrystalline hydroxyapatite paste ( NHA ) into fresh extraction sockets in dogs .
	manualset3
140707	6	408627	5	NULL	NULL	0	NULL	nanocrystalline hydroxyapatite paste ( NHA ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to evaluate the histological response and dimensional ridge alterations following application of a nanocrystalline hydroxyapatite paste ( NHA ) into fresh extraction sockets in dogs .
	manualset3
140708	7	408627	5	NULL	NULL	0	NULL	fresh extraction sockets 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to evaluate the histological response and dimensional ridge alterations following application of a nanocrystalline hydroxyapatite paste ( NHA ) into fresh extraction sockets in dogs .
	manualset3
140709	8	408627	5	NULL	NULL	0	NULL	dogs 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to evaluate the histological response and dimensional ridge alterations following application of a nanocrystalline hydroxyapatite paste ( NHA ) into fresh extraction sockets in dogs .
	manualset3
140710	1	408628	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to investigate the presence of dysphagia in patients with genetically proven DM2 who reported difficulty in swallowing for solid food at the questionnaire survey .
	manualset3
140711	2	408628	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to investigate the presence of dysphagia in patients with genetically proven DM2 who reported difficulty in swallowing for solid food at the questionnaire survey .
	manualset3
140712	3	408628	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to investigate the presence of dysphagia in patients with genetically proven DM2 who reported difficulty in swallowing for solid food at the questionnaire survey .
	manualset3
140713	4	408628	5	NULL	NULL	0	NULL	dysphagia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to investigate the presence of dysphagia in patients with genetically proven DM2 who reported difficulty in swallowing for solid food at the questionnaire survey .
	manualset3
140714	5	408628	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to investigate the presence of dysphagia in patients with genetically proven DM2 who reported difficulty in swallowing for solid food at the questionnaire survey .
	manualset3
140715	6	408628	5	NULL	NULL	0	NULL	 genetically proven DM2	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to investigate the presence of dysphagia in patients with genetically proven DM2 who reported difficulty in swallowing for solid food at the questionnaire survey .
	manualset3
140716	7	408628	5	NULL	NULL	0	NULL	difficulty in swallowing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to investigate the presence of dysphagia in patients with genetically proven DM2 who reported difficulty in swallowing for solid food at the questionnaire survey .
	manualset3
140717	8	408628	5	NULL	NULL	0	NULL	solid food	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to investigate the presence of dysphagia in patients with genetically proven DM2 who reported difficulty in swallowing for solid food at the questionnaire survey .
	manualset3
140718	9	408628	5	NULL	NULL	0	NULL	questionnaire survey	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study was to investigate the presence of dysphagia in patients with genetically proven DM2 who reported difficulty in swallowing for solid food at the questionnaire survey .
	manualset3
140719	1	408629	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the work was to establish the frequency of convulsion recurrence through the retrospective study with regard to age , type of recurrence , and applied prophylaxis in children in Tuzla Canton in a two-year period after the first febrile convulsion .
	manualset3
140720	2	408629	5	NULL	NULL	0	NULL	frequency 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the work was to establish the frequency of convulsion recurrence through the retrospective study with regard to age , type of recurrence , and applied prophylaxis in children in Tuzla Canton in a two-year period after the first febrile convulsion .
	manualset3
140721	3	408629	5	NULL	NULL	0	NULL	convulsion recurrence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the work was to establish the frequency of convulsion recurrence through the retrospective study with regard to age , type of recurrence , and applied prophylaxis in children in Tuzla Canton in a two-year period after the first febrile convulsion .
	manualset3
140722	4	408629	5	NULL	NULL	0	NULL	retrospective study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the work was to establish the frequency of convulsion recurrence through the retrospective study with regard to age , type of recurrence , and applied prophylaxis in children in Tuzla Canton in a two-year period after the first febrile convulsion .
	manualset3
140723	5	408629	5	NULL	NULL	0	NULL	age 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the work was to establish the frequency of convulsion recurrence through the retrospective study with regard to age , type of recurrence , and applied prophylaxis in children in Tuzla Canton in a two-year period after the first febrile convulsion .
	manualset3
140724	6	408629	5	NULL	NULL	0	NULL	 type of recurrence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the work was to establish the frequency of convulsion recurrence through the retrospective study with regard to age , type of recurrence , and applied prophylaxis in children in Tuzla Canton in a two-year period after the first febrile convulsion .
	manualset3
140725	7	408629	5	NULL	NULL	0	NULL	prophylaxis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the work was to establish the frequency of convulsion recurrence through the retrospective study with regard to age , type of recurrence , and applied prophylaxis in children in Tuzla Canton in a two-year period after the first febrile convulsion .
	manualset3
140726	8	408629	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the work was to establish the frequency of convulsion recurrence through the retrospective study with regard to age , type of recurrence , and applied prophylaxis in children in Tuzla Canton in a two-year period after the first febrile convulsion .
	manualset3
140727	9	408629	5	NULL	NULL	0	NULL	Tuzla Canton	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the work was to establish the frequency of convulsion recurrence through the retrospective study with regard to age , type of recurrence , and applied prophylaxis in children in Tuzla Canton in a two-year period after the first febrile convulsion .
	manualset3
140728	10	408629	5	NULL	NULL	0	NULL	two-year period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the work was to establish the frequency of convulsion recurrence through the retrospective study with regard to age , type of recurrence , and applied prophylaxis in children in Tuzla Canton in a two-year period after the first febrile convulsion .
	manualset3
140729	11	408629	5	NULL	NULL	0	NULL	first febrile convulsion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the work was to establish the frequency of convulsion recurrence through the retrospective study with regard to age , type of recurrence , and applied prophylaxis in children in Tuzla Canton in a two-year period after the first febrile convulsion .
	manualset3
142899	12	408629	5	NULL	NULL	0	NULL	work 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the work was to establish the frequency of convulsion recurrence through the retrospective study with regard to age , type of recurrence , and applied prophylaxis in children in Tuzla Canton in a two-year period after the first febrile convulsion .
	manualset3
140730	1	408630	5	NULL	NULL	0	NULL	aim	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of therapy was obliteration of distal esophageal varices by EVL , every 2 to 4 weeks , until eradication .
	manualset3
140731	2	408630	5	NULL	NULL	NULL	NULL	therapy 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The aim of therapy was obliteration of distal esophageal varices by EVL , every 2 to 4 weeks , until eradication .
	manualset3
140732	3	408630	5	NULL	NULL	NULL	NULL	obliteration 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The aim of therapy was obliteration of distal esophageal varices by EVL , every 2 to 4 weeks , until eradication .
	manualset3
140733	4	408630	5	NULL	NULL	0	NULL	distal esophageal varices 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of therapy was obliteration of distal esophageal varices by EVL , every 2 to 4 weeks , until eradication .
	manualset3
140734	5	408630	5	NULL	NULL	0	NULL	EVL 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of therapy was obliteration of distal esophageal varices by EVL , every 2 to 4 weeks , until eradication .
	manualset3
140735	6	408630	5	NULL	NULL	0	NULL	 2 to 4 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of therapy was obliteration of distal esophageal varices by EVL , every 2 to 4 weeks , until eradication .
	manualset3
140736	7	408630	5	NULL	NULL	0	NULL	eradication 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of therapy was obliteration of distal esophageal varices by EVL , every 2 to 4 weeks , until eradication .
	manualset3
140737	1	408631	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this article is to discuss different methods of assessing dry weight and to determine their role in the complex fluid management of end-stage renal disease patient .
	manualset3
140738	2	408631	5	NULL	NULL	0	NULL	article 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this article is to discuss different methods of assessing dry weight and to determine their role in the complex fluid management of end-stage renal disease patient .
	manualset3
140739	3	408631	5	NULL	NULL	0	NULL	methods 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this article is to discuss different methods of assessing dry weight and to determine their role in the complex fluid management of end-stage renal disease patient .
	manualset3
140740	4	408631	5	NULL	NULL	0	NULL	dry weight 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this article is to discuss different methods of assessing dry weight and to determine their role in the complex fluid management of end-stage renal disease patient .
	manualset3
140741	5	408631	5	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this article is to discuss different methods of assessing dry weight and to determine their role in the complex fluid management of end-stage renal disease patient .
	manualset3
140742	6	408631	5	NULL	NULL	0	NULL	complex fluid management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this article is to discuss different methods of assessing dry weight and to determine their role in the complex fluid management of end-stage renal disease patient .
	manualset3
140743	7	408631	5	NULL	NULL	0	NULL	end-stage renal disease patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this article is to discuss different methods of assessing dry weight and to determine their role in the complex fluid management of end-stage renal disease patient .
	manualset3
140744	1	408632	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this investigation was to explore the relative importance of psychologic variables in explaining the degree of denture satisfaction in full denture patients .
	manualset3
140745	2	408632	5	NULL	NULL	0	NULL	investigation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this investigation was to explore the relative importance of psychologic variables in explaining the degree of denture satisfaction in full denture patients .
	manualset3
140746	3	408632	5	NULL	NULL	0	NULL	relative importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this investigation was to explore the relative importance of psychologic variables in explaining the degree of denture satisfaction in full denture patients .
	manualset3
140747	4	408632	5	NULL	NULL	0	NULL	psychologic variables	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this investigation was to explore the relative importance of psychologic variables in explaining the degree of denture satisfaction in full denture patients .
	manualset3
140748	5	408632	5	NULL	NULL	NULL	NULL	degree of denture satisfaction	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The aim of this investigation was to explore the relative importance of psychologic variables in explaining the degree of denture satisfaction in full denture patients .
	manualset3
140749	6	408632	5	NULL	NULL	0	NULL	denture patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this investigation was to explore the relative importance of psychologic variables in explaining the degree of denture satisfaction in full denture patients .
	manualset3
140750	1	408633	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this paper is to look upon the use of social media in relevant professional communities in the light of the HENVINET experience , and to reflect on the acceptance and usefulness of such a new approach .
	manualset3
140751	2	408633	5	NULL	NULL	0	NULL	paper 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this paper is to look upon the use of social media in relevant professional communities in the light of the HENVINET experience , and to reflect on the acceptance and usefulness of such a new approach .
	manualset3
140752	3	408633	5	NULL	NULL	0	NULL	social media	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this paper is to look upon the use of social media in relevant professional communities in the light of the HENVINET experience , and to reflect on the acceptance and usefulness of such a new approach .
	manualset3
140753	4	408633	5	NULL	NULL	0	NULL	professional communities	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this paper is to look upon the use of social media in relevant professional communities in the light of the HENVINET experience , and to reflect on the acceptance and usefulness of such a new approach .
	manualset3
140754	5	408633	5	NULL	NULL	0	NULL	HENVINET experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this paper is to look upon the use of social media in relevant professional communities in the light of the HENVINET experience , and to reflect on the acceptance and usefulness of such a new approach .
	manualset3
140755	6	408633	5	NULL	NULL	0	NULL	acceptance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this paper is to look upon the use of social media in relevant professional communities in the light of the HENVINET experience , and to reflect on the acceptance and usefulness of such a new approach .
	manualset3
140756	7	408633	5	NULL	NULL	0	NULL	usefulness 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this paper is to look upon the use of social media in relevant professional communities in the light of the HENVINET experience , and to reflect on the acceptance and usefulness of such a new approach .
	manualset3
144835	8	408633	5	NULL	NULL	0	NULL	approach 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this paper is to look upon the use of social media in relevant professional communities in the light of the HENVINET experience , and to reflect on the acceptance and usefulness of such a new approach .
	manualset3
140757	1	408634	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this paper was assessment of usefulness of MPPW recording in diagnosis of hearing loss .
	manualset3
140758	2	408634	5	NULL	NULL	0	NULL	paper 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this paper was assessment of usefulness of MPPW recording in diagnosis of hearing loss .
	manualset3
140759	3	408634	5	NULL	NULL	0	NULL	usefulness 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this paper was assessment of usefulness of MPPW recording in diagnosis of hearing loss .
	manualset3
140760	4	408634	5	NULL	NULL	0	NULL	MPPW recording	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this paper was assessment of usefulness of MPPW recording in diagnosis of hearing loss .
	manualset3
140761	5	408634	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this paper was assessment of usefulness of MPPW recording in diagnosis of hearing loss .
	manualset3
140762	6	408634	5	NULL	NULL	0	NULL	hearing loss	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this paper was assessment of usefulness of MPPW recording in diagnosis of hearing loss .
	manualset3
140763	1	408635	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this paper was to validate an analytical method for the simultaneous determination of PTX and its active metabolite ( - ) - ( R ) - M1 in rat serum and some tissues using a high-performance liquid chromatography method with ultraviolet detection ( HPLC-UV ) .
	manualset3
140764	2	408635	5	NULL	NULL	0	NULL	paper 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this paper was to validate an analytical method for the simultaneous determination of PTX and its active metabolite ( - ) - ( R ) - M1 in rat serum and some tissues using a high-performance liquid chromatography method with ultraviolet detection ( HPLC-UV ) .
	manualset3
140765	3	408635	5	NULL	NULL	0	NULL	analytical method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this paper was to validate an analytical method for the simultaneous determination of PTX and its active metabolite ( - ) - ( R ) - M1 in rat serum and some tissues using a high-performance liquid chromatography method with ultraviolet detection ( HPLC-UV ) .
	manualset3
140766	4	408635	5	NULL	NULL	0	NULL	determination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this paper was to validate an analytical method for the simultaneous determination of PTX and its active metabolite ( - ) - ( R ) - M1 in rat serum and some tissues using a high-performance liquid chromatography method with ultraviolet detection ( HPLC-UV ) .
	manualset3
140767	5	408635	5	NULL	NULL	0	NULL	PTX 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this paper was to validate an analytical method for the simultaneous determination of PTX and its active metabolite ( - ) - ( R ) - M1 in rat serum and some tissues using a high-performance liquid chromatography method with ultraviolet detection ( HPLC-UV ) .
	manualset3
140768	6	408635	5	NULL	NULL	0	NULL	active metabolite ( - ) - ( R ) - M1	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this paper was to validate an analytical method for the simultaneous determination of PTX and its active metabolite ( - ) - ( R ) - M1 in rat serum and some tissues using a high-performance liquid chromatography method with ultraviolet detection ( HPLC-UV ) .
	manualset3
140769	7	408635	5	NULL	NULL	0	NULL	rat serum	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this paper was to validate an analytical method for the simultaneous determination of PTX and its active metabolite ( - ) - ( R ) - M1 in rat serum and some tissues using a high-performance liquid chromatography method with ultraviolet detection ( HPLC-UV ) .
	manualset3
140770	8	408635	5	NULL	NULL	0	NULL	tissues 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this paper was to validate an analytical method for the simultaneous determination of PTX and its active metabolite ( - ) - ( R ) - M1 in rat serum and some tissues using a high-performance liquid chromatography method with ultraviolet detection ( HPLC-UV ) .
	manualset3
140771	9	408635	5	NULL	NULL	NULL	NULL	high-performance liquid chromatography method with ultraviolet detection ( HPLC-UV )	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The aim of this paper was to validate an analytical method for the simultaneous determination of PTX and its active metabolite ( - ) - ( R ) - M1 in rat serum and some tissues using a high-performance liquid chromatography method with ultraviolet detection ( HPLC-UV ) .
	manualset3
140772	1	408636	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this pilot study was to determine VEGF serum levels ( S-VEGF ) at diagnosis and at restaging in children diagnosed with cancer , and to investigate whether this parameter provides prognostic information for remission after induction therapy and response to treatment .
	manualset3
140773	2	408636	5	NULL	NULL	0	NULL	pilot study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this pilot study was to determine VEGF serum levels ( S-VEGF ) at diagnosis and at restaging in children diagnosed with cancer , and to investigate whether this parameter provides prognostic information for remission after induction therapy and response to treatment .
	manualset3
140774	3	408636	5	NULL	NULL	0	NULL	VEGF serum levels ( S-VEGF )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this pilot study was to determine VEGF serum levels ( S-VEGF ) at diagnosis and at restaging in children diagnosed with cancer , and to investigate whether this parameter provides prognostic information for remission after induction therapy and response to treatment .
	manualset3
140775	4	408636	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this pilot study was to determine VEGF serum levels ( S-VEGF ) at diagnosis and at restaging in children diagnosed with cancer , and to investigate whether this parameter provides prognostic information for remission after induction therapy and response to treatment .
	manualset3
140776	5	408636	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this pilot study was to determine VEGF serum levels ( S-VEGF ) at diagnosis and at restaging in children diagnosed with cancer , and to investigate whether this parameter provides prognostic information for remission after induction therapy and response to treatment .
	manualset3
140777	6	408636	5	NULL	NULL	0	NULL	cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this pilot study was to determine VEGF serum levels ( S-VEGF ) at diagnosis and at restaging in children diagnosed with cancer , and to investigate whether this parameter provides prognostic information for remission after induction therapy and response to treatment .
	manualset3
140778	7	408636	5	NULL	NULL	0	NULL	parameter 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this pilot study was to determine VEGF serum levels ( S-VEGF ) at diagnosis and at restaging in children diagnosed with cancer , and to investigate whether this parameter provides prognostic information for remission after induction therapy and response to treatment .
	manualset3
140779	8	408636	5	NULL	NULL	0	NULL	prognostic information	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this pilot study was to determine VEGF serum levels ( S-VEGF ) at diagnosis and at restaging in children diagnosed with cancer , and to investigate whether this parameter provides prognostic information for remission after induction therapy and response to treatment .
	manualset3
140780	9	408636	5	NULL	NULL	NULL	NULL	remission	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The aim of this pilot study was to determine VEGF serum levels ( S-VEGF ) at diagnosis and at restaging in children diagnosed with cancer , and to investigate whether this parameter provides prognostic information for remission after induction therapy and response to treatment .
	manualset3
140781	10	408636	5	NULL	NULL	0	NULL	induction therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this pilot study was to determine VEGF serum levels ( S-VEGF ) at diagnosis and at restaging in children diagnosed with cancer , and to investigate whether this parameter provides prognostic information for remission after induction therapy and response to treatment .
	manualset3
140782	11	408636	5	NULL	NULL	0	NULL	response 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this pilot study was to determine VEGF serum levels ( S-VEGF ) at diagnosis and at restaging in children diagnosed with cancer , and to investigate whether this parameter provides prognostic information for remission after induction therapy and response to treatment .
	manualset3
140783	12	408636	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this pilot study was to determine VEGF serum levels ( S-VEGF ) at diagnosis and at restaging in children diagnosed with cancer , and to investigate whether this parameter provides prognostic information for remission after induction therapy and response to treatment .
	manualset3
140784	1	408637	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this project is to develop a common homeopathic terminology to improve communication .
	manualset3
140785	2	408637	5	NULL	NULL	0	NULL	project 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this project is to develop a common homeopathic terminology to improve communication .
	manualset3
140786	3	408637	5	NULL	NULL	0	NULL	common homeopathic terminology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this project is to develop a common homeopathic terminology to improve communication .
	manualset3
140787	4	408637	5	NULL	NULL	0	NULL	communication 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this project is to develop a common homeopathic terminology to improve communication .
	manualset3
140788	1	408638	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this research is to study the effect of neodymium ion on the cell wall structure of Staphyloccocus aruea using transmission electron microscope , amino acid analyzer , infrared absorption spectrometry ( IR ) .
	manualset3
140789	2	408638	5	NULL	NULL	0	NULL	research 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this research is to study the effect of neodymium ion on the cell wall structure of Staphyloccocus aruea using transmission electron microscope , amino acid analyzer , infrared absorption spectrometry ( IR ) .
	manualset3
140790	3	408638	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this research is to study the effect of neodymium ion on the cell wall structure of Staphyloccocus aruea using transmission electron microscope , amino acid analyzer , infrared absorption spectrometry ( IR ) .
	manualset3
140791	4	408638	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this research is to study the effect of neodymium ion on the cell wall structure of Staphyloccocus aruea using transmission electron microscope , amino acid analyzer , infrared absorption spectrometry ( IR ) .
	manualset3
140792	5	408638	5	NULL	NULL	0	NULL	neodymium ion	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this research is to study the effect of neodymium ion on the cell wall structure of Staphyloccocus aruea using transmission electron microscope , amino acid analyzer , infrared absorption spectrometry ( IR ) .
	manualset3
140793	6	408638	5	NULL	NULL	0	NULL	cell wall structure 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this research is to study the effect of neodymium ion on the cell wall structure of Staphyloccocus aruea using transmission electron microscope , amino acid analyzer , infrared absorption spectrometry ( IR ) .
	manualset3
140794	7	408638	5	NULL	NULL	0	NULL	Staphyloccocus aruea	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this research is to study the effect of neodymium ion on the cell wall structure of Staphyloccocus aruea using transmission electron microscope , amino acid analyzer , infrared absorption spectrometry ( IR ) .
	manualset3
140795	8	408638	5	NULL	NULL	0	NULL	transmission electron microscope	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this research is to study the effect of neodymium ion on the cell wall structure of Staphyloccocus aruea using transmission electron microscope , amino acid analyzer , infrared absorption spectrometry ( IR ) .
	manualset3
140796	9	408638	5	NULL	NULL	0	NULL	amino acid analyzer	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this research is to study the effect of neodymium ion on the cell wall structure of Staphyloccocus aruea using transmission electron microscope , amino acid analyzer , infrared absorption spectrometry ( IR ) .
	manualset3
140797	10	408638	5	NULL	NULL	0	NULL	infrared absorption spectrometry ( IR )	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this research is to study the effect of neodymium ion on the cell wall structure of Staphyloccocus aruea using transmission electron microscope , amino acid analyzer , infrared absorption spectrometry ( IR ) .
	manualset3
140798	1	408639	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this review is considering available literature on endocrine roles of NO and/or its metabolites , i.e. nitrite and nitrate .
	manualset3
140799	2	408639	5	NULL	NULL	0	NULL	review 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this review is considering available literature on endocrine roles of NO and/or its metabolites , i.e. nitrite and nitrate .
	manualset3
140800	3	408639	5	NULL	NULL	0	NULL	literature 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this review is considering available literature on endocrine roles of NO and/or its metabolites , i.e. nitrite and nitrate .
	manualset3
140801	4	408639	5	NULL	NULL	0	NULL	endocrine roles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this review is considering available literature on endocrine roles of NO and/or its metabolites , i.e. nitrite and nitrate .
	manualset3
140802	5	408639	5	NULL	NULL	0	NULL	NO 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this review is considering available literature on endocrine roles of NO and/or its metabolites , i.e. nitrite and nitrate .
	manualset3
140803	6	408639	5	NULL	NULL	0	NULL	metabolites 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this review is considering available literature on endocrine roles of NO and/or its metabolites , i.e. nitrite and nitrate .
	manualset3
140804	7	408639	5	NULL	NULL	0	NULL	nitrite 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this review is considering available literature on endocrine roles of NO and/or its metabolites , i.e. nitrite and nitrate .
	manualset3
140805	8	408639	5	NULL	NULL	0	NULL	nitrate 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this review is considering available literature on endocrine roles of NO and/or its metabolites , i.e. nitrite and nitrate .
	manualset3
140806	1	408640	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this review is to examine the current scientific knowledge on the relationship between diet and Type 2 diabetes and consider further implications for public health .
	manualset3
140807	2	408640	5	NULL	NULL	0	NULL	review 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this review is to examine the current scientific knowledge on the relationship between diet and Type 2 diabetes and consider further implications for public health .
	manualset3
140808	3	408640	5	NULL	NULL	0	NULL	current scientific knowledge	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this review is to examine the current scientific knowledge on the relationship between diet and Type 2 diabetes and consider further implications for public health .
	manualset3
140809	4	408640	5	NULL	NULL	0	NULL	relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this review is to examine the current scientific knowledge on the relationship between diet and Type 2 diabetes and consider further implications for public health .
	manualset3
140810	5	408640	5	NULL	NULL	0	NULL	diet 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this review is to examine the current scientific knowledge on the relationship between diet and Type 2 diabetes and consider further implications for public health .
	manualset3
140811	6	408640	5	NULL	NULL	0	NULL	Type 2 diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this review is to examine the current scientific knowledge on the relationship between diet and Type 2 diabetes and consider further implications for public health .
	manualset3
140812	7	408640	5	NULL	NULL	0	NULL	implications 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this review is to examine the current scientific knowledge on the relationship between diet and Type 2 diabetes and consider further implications for public health .
	manualset3
140813	8	408640	5	NULL	NULL	0	NULL	public health	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this review is to examine the current scientific knowledge on the relationship between diet and Type 2 diabetes and consider further implications for public health .
	manualset3
140814	1	408641	5	NULL	NULL	0	NULL	Chemotherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Chemotherapy of non-Hodgkin lymphomas ) .
	manualset3
140815	2	408641	5	NULL	NULL	0	NULL	non-Hodgkin lymphomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Chemotherapy of non-Hodgkin lymphomas ) .
	manualset3
140816	1	408642	5	NULL	NULL	NULL	NULL	reversed-phase high-performance liquid chromatography ( HPLC ) method	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A reversed-phase high-performance liquid chromatography ( HPLC ) method with ultraviolet ( UV ) detection at 318nm was carried out on a C18 column , using a mixture of potassium dihydrogen phosphate buffer , acetonitrile , and methanol ( 55 : 15 : 30 , v/v/v ) as a mobile phase with a flow rate of 1.0 ml/min .
	manualset3
140817	2	408642	5	NULL	NULL	0	NULL	ultraviolet ( UV ) detection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A reversed-phase high-performance liquid chromatography ( HPLC ) method with ultraviolet ( UV ) detection at 318nm was carried out on a C18 column , using a mixture of potassium dihydrogen phosphate buffer , acetonitrile , and methanol ( 55 : 15 : 30 , v/v/v ) as a mobile phase with a flow rate of 1.0 ml/min .
	manualset3
140818	3	408642	5	NULL	NULL	0	NULL	318nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A reversed-phase high-performance liquid chromatography ( HPLC ) method with ultraviolet ( UV ) detection at 318nm was carried out on a C18 column , using a mixture of potassium dihydrogen phosphate buffer , acetonitrile , and methanol ( 55 : 15 : 30 , v/v/v ) as a mobile phase with a flow rate of 1.0 ml/min .
	manualset3
140819	4	408642	5	NULL	NULL	0	NULL	C18 column	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A reversed-phase high-performance liquid chromatography ( HPLC ) method with ultraviolet ( UV ) detection at 318nm was carried out on a C18 column , using a mixture of potassium dihydrogen phosphate buffer , acetonitrile , and methanol ( 55 : 15 : 30 , v/v/v ) as a mobile phase with a flow rate of 1.0 ml/min .
	manualset3
140820	5	408642	5	NULL	NULL	0	NULL	mixture 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A reversed-phase high-performance liquid chromatography ( HPLC ) method with ultraviolet ( UV ) detection at 318nm was carried out on a C18 column , using a mixture of potassium dihydrogen phosphate buffer , acetonitrile , and methanol ( 55 : 15 : 30 , v/v/v ) as a mobile phase with a flow rate of 1.0 ml/min .
	manualset3
140821	6	408642	5	NULL	NULL	0	NULL	potassium dihydrogen phosphate buffer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A reversed-phase high-performance liquid chromatography ( HPLC ) method with ultraviolet ( UV ) detection at 318nm was carried out on a C18 column , using a mixture of potassium dihydrogen phosphate buffer , acetonitrile , and methanol ( 55 : 15 : 30 , v/v/v ) as a mobile phase with a flow rate of 1.0 ml/min .
	manualset3
140822	7	408642	5	NULL	NULL	0	NULL	acetonitrile 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A reversed-phase high-performance liquid chromatography ( HPLC ) method with ultraviolet ( UV ) detection at 318nm was carried out on a C18 column , using a mixture of potassium dihydrogen phosphate buffer , acetonitrile , and methanol ( 55 : 15 : 30 , v/v/v ) as a mobile phase with a flow rate of 1.0 ml/min .
	manualset3
140823	8	408642	5	NULL	NULL	0	NULL	methanol 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A reversed-phase high-performance liquid chromatography ( HPLC ) method with ultraviolet ( UV ) detection at 318nm was carried out on a C18 column , using a mixture of potassium dihydrogen phosphate buffer , acetonitrile , and methanol ( 55 : 15 : 30 , v/v/v ) as a mobile phase with a flow rate of 1.0 ml/min .
	manualset3
140824	9	408642	5	NULL	NULL	0	NULL	55 : 15 : 30 , v/v/v 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A reversed-phase high-performance liquid chromatography ( HPLC ) method with ultraviolet ( UV ) detection at 318nm was carried out on a C18 column , using a mixture of potassium dihydrogen phosphate buffer , acetonitrile , and methanol ( 55 : 15 : 30 , v/v/v ) as a mobile phase with a flow rate of 1.0 ml/min .
	manualset3
140825	10	408642	5	NULL	NULL	0	NULL	mobile phase	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A reversed-phase high-performance liquid chromatography ( HPLC ) method with ultraviolet ( UV ) detection at 318nm was carried out on a C18 column , using a mixture of potassium dihydrogen phosphate buffer , acetonitrile , and methanol ( 55 : 15 : 30 , v/v/v ) as a mobile phase with a flow rate of 1.0 ml/min .
	manualset3
140826	11	408642	5	NULL	NULL	0	NULL	flow rate 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A reversed-phase high-performance liquid chromatography ( HPLC ) method with ultraviolet ( UV ) detection at 318nm was carried out on a C18 column , using a mixture of potassium dihydrogen phosphate buffer , acetonitrile , and methanol ( 55 : 15 : 30 , v/v/v ) as a mobile phase with a flow rate of 1.0 ml/min .
	manualset3
140827	12	408642	5	NULL	NULL	0	NULL	1.0 ml/min	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A reversed-phase high-performance liquid chromatography ( HPLC ) method with ultraviolet ( UV ) detection at 318nm was carried out on a C18 column , using a mixture of potassium dihydrogen phosphate buffer , acetonitrile , and methanol ( 55 : 15 : 30 , v/v/v ) as a mobile phase with a flow rate of 1.0 ml/min .
	manualset3
140828	1	408643	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this review is to provide current status on the search for an accurate plasma biomarker for acute mesenteric ischemia .
	manualset3
140829	2	408643	5	NULL	NULL	0	NULL	review 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this review is to provide current status on the search for an accurate plasma biomarker for acute mesenteric ischemia .
	manualset3
140830	3	408643	5	NULL	NULL	0	NULL	current status	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this review is to provide current status on the search for an accurate plasma biomarker for acute mesenteric ischemia .
	manualset3
140831	4	408643	5	NULL	NULL	0	NULL	plasma biomarker	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this review is to provide current status on the search for an accurate plasma biomarker for acute mesenteric ischemia .
	manualset3
140832	5	408643	5	NULL	NULL	0	NULL	acute mesenteric ischemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this review is to provide current status on the search for an accurate plasma biomarker for acute mesenteric ischemia .
	manualset3
140833	1	408644	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study , therefore , was to investigate the genotoxic and biokinetics consequences of exposure to depleted insoluble uranium dioxide ( UO2 ) by repeated or acute inhalation on subsequent acute inhalation of moderately soluble uranium peroxide ( UO4 ) in rats .
	manualset3
140834	2	408644	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study , therefore , was to investigate the genotoxic and biokinetics consequences of exposure to depleted insoluble uranium dioxide ( UO2 ) by repeated or acute inhalation on subsequent acute inhalation of moderately soluble uranium peroxide ( UO4 ) in rats .
	manualset3
140835	3	408644	5	NULL	NULL	0	NULL	genotoxic consequences 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study , therefore , was to investigate the genotoxic and biokinetics consequences of exposure to depleted insoluble uranium dioxide ( UO2 ) by repeated or acute inhalation on subsequent acute inhalation of moderately soluble uranium peroxide ( UO4 ) in rats .
	manualset3
140836	4	408644	5	NULL	NULL	0	NULL	biokinetics consequences 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study , therefore , was to investigate the genotoxic and biokinetics consequences of exposure to depleted insoluble uranium dioxide ( UO2 ) by repeated or acute inhalation on subsequent acute inhalation of moderately soluble uranium peroxide ( UO4 ) in rats .
	manualset3
140837	5	408644	5	NULL	NULL	0	NULL	exposure 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study , therefore , was to investigate the genotoxic and biokinetics consequences of exposure to depleted insoluble uranium dioxide ( UO2 ) by repeated or acute inhalation on subsequent acute inhalation of moderately soluble uranium peroxide ( UO4 ) in rats .
	manualset3
140838	6	408644	5	NULL	NULL	0	NULL	uranium dioxide ( UO2 ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study , therefore , was to investigate the genotoxic and biokinetics consequences of exposure to depleted insoluble uranium dioxide ( UO2 ) by repeated or acute inhalation on subsequent acute inhalation of moderately soluble uranium peroxide ( UO4 ) in rats .
	manualset3
140839	7	408644	5	NULL	NULL	0	NULL	repeated or acute inhalation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study , therefore , was to investigate the genotoxic and biokinetics consequences of exposure to depleted insoluble uranium dioxide ( UO2 ) by repeated or acute inhalation on subsequent acute inhalation of moderately soluble uranium peroxide ( UO4 ) in rats .
	manualset3
140840	8	408644	5	NULL	NULL	0	NULL	subsequent acute inhalation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study , therefore , was to investigate the genotoxic and biokinetics consequences of exposure to depleted insoluble uranium dioxide ( UO2 ) by repeated or acute inhalation on subsequent acute inhalation of moderately soluble uranium peroxide ( UO4 ) in rats .
	manualset3
140841	9	408644	5	NULL	NULL	0	NULL	 uranium peroxide ( UO4 )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study , therefore , was to investigate the genotoxic and biokinetics consequences of exposure to depleted insoluble uranium dioxide ( UO2 ) by repeated or acute inhalation on subsequent acute inhalation of moderately soluble uranium peroxide ( UO4 ) in rats .
	manualset3
140842	10	408644	5	NULL	NULL	0	NULL	rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study , therefore , was to investigate the genotoxic and biokinetics consequences of exposure to depleted insoluble uranium dioxide ( UO2 ) by repeated or acute inhalation on subsequent acute inhalation of moderately soluble uranium peroxide ( UO4 ) in rats .
	manualset3
140843	1	408645	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to clarify the usefulness of defect reperfusion ultrasound ( US ) imaging using Sonazoid in the management of hepatocellular carcinoma ( HCC ) .
	manualset3
140844	2	408645	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to clarify the usefulness of defect reperfusion ultrasound ( US ) imaging using Sonazoid in the management of hepatocellular carcinoma ( HCC ) .
	manualset3
140845	3	408645	5	NULL	NULL	0	NULL	usefulness 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to clarify the usefulness of defect reperfusion ultrasound ( US ) imaging using Sonazoid in the management of hepatocellular carcinoma ( HCC ) .
	manualset3
140846	4	408645	5	NULL	NULL	0	NULL	reperfusion ultrasound ( US ) imaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to clarify the usefulness of defect reperfusion ultrasound ( US ) imaging using Sonazoid in the management of hepatocellular carcinoma ( HCC ) .
	manualset3
140847	5	408645	5	NULL	NULL	0	NULL	Sonazoid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to clarify the usefulness of defect reperfusion ultrasound ( US ) imaging using Sonazoid in the management of hepatocellular carcinoma ( HCC ) .
	manualset3
140848	6	408645	5	NULL	NULL	0	NULL	management 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to clarify the usefulness of defect reperfusion ultrasound ( US ) imaging using Sonazoid in the management of hepatocellular carcinoma ( HCC ) .
	manualset3
140849	7	408645	5	NULL	NULL	0	NULL	hepatocellular carcinoma ( HCC )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to clarify the usefulness of defect reperfusion ultrasound ( US ) imaging using Sonazoid in the management of hepatocellular carcinoma ( HCC ) .
	manualset3
140850	1	408646	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to develop a prototype system for noncontact , noninvasive and unconstrained vital sign monitoring using microwave radar and to use the system to measure the respiratory rate of a Japanese black bear ( Ursus thibetanus japonicus ) during hibernation for ensuring the bear 's safety .
	manualset3
140851	2	408646	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to develop a prototype system for noncontact , noninvasive and unconstrained vital sign monitoring using microwave radar and to use the system to measure the respiratory rate of a Japanese black bear ( Ursus thibetanus japonicus ) during hibernation for ensuring the bear 's safety .
	manualset3
140852	3	408646	5	NULL	NULL	0	NULL	prototype system	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to develop a prototype system for noncontact , noninvasive and unconstrained vital sign monitoring using microwave radar and to use the system to measure the respiratory rate of a Japanese black bear ( Ursus thibetanus japonicus ) during hibernation for ensuring the bear 's safety .
	manualset3
140853	4	408646	5	NULL	NULL	0	NULL	microwave radar 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to develop a prototype system for noncontact , noninvasive and unconstrained vital sign monitoring using microwave radar and to use the system to measure the respiratory rate of a Japanese black bear ( Ursus thibetanus japonicus ) during hibernation for ensuring the bear 's safety .
	manualset3
140854	5	408646	5	NULL	NULL	0	NULL	system 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to develop a prototype system for noncontact , noninvasive and unconstrained vital sign monitoring using microwave radar and to use the system to measure the respiratory rate of a Japanese black bear ( Ursus thibetanus japonicus ) during hibernation for ensuring the bear 's safety .
	manualset3
140855	6	408646	5	NULL	NULL	0	NULL	respiratory rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to develop a prototype system for noncontact , noninvasive and unconstrained vital sign monitoring using microwave radar and to use the system to measure the respiratory rate of a Japanese black bear ( Ursus thibetanus japonicus ) during hibernation for ensuring the bear 's safety .
	manualset3
140856	7	408646	5	NULL	NULL	0	NULL	Japanese black bear ( Ursus thibetanus japonicus )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to develop a prototype system for noncontact , noninvasive and unconstrained vital sign monitoring using microwave radar and to use the system to measure the respiratory rate of a Japanese black bear ( Ursus thibetanus japonicus ) during hibernation for ensuring the bear 's safety .
	manualset3
140857	8	408646	5	NULL	NULL	0	NULL	hibernation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to develop a prototype system for noncontact , noninvasive and unconstrained vital sign monitoring using microwave radar and to use the system to measure the respiratory rate of a Japanese black bear ( Ursus thibetanus japonicus ) during hibernation for ensuring the bear 's safety .
	manualset3
140858	9	408646	5	NULL	NULL	0	NULL	safety 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to develop a prototype system for noncontact , noninvasive and unconstrained vital sign monitoring using microwave radar and to use the system to measure the respiratory rate of a Japanese black bear ( Ursus thibetanus japonicus ) during hibernation for ensuring the bear 's safety .
	manualset3
144836	10	408646	5	NULL	NULL	0	NULL	vital sign monitoring	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to develop a prototype system for noncontact , noninvasive and unconstrained vital sign monitoring using microwave radar and to use the system to measure the respiratory rate of a Japanese black bear ( Ursus thibetanus japonicus ) during hibernation for ensuring the bear 's safety .
	manualset3
140859	1	408647	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to evaluate the role of desferrioxamine in the prevention of pancreatic injury following major hepatectomy .
	manualset3
140860	2	408647	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to evaluate the role of desferrioxamine in the prevention of pancreatic injury following major hepatectomy .
	manualset3
140861	3	408647	5	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to evaluate the role of desferrioxamine in the prevention of pancreatic injury following major hepatectomy .
	manualset3
140862	4	408647	5	NULL	NULL	0	NULL	desferrioxamine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to evaluate the role of desferrioxamine in the prevention of pancreatic injury following major hepatectomy .
	manualset3
140863	5	408647	5	NULL	NULL	0	NULL	prevention 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to evaluate the role of desferrioxamine in the prevention of pancreatic injury following major hepatectomy .
	manualset3
140864	6	408647	5	NULL	NULL	0	NULL	pancreatic injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to evaluate the role of desferrioxamine in the prevention of pancreatic injury following major hepatectomy .
	manualset3
140865	7	408647	5	NULL	NULL	0	NULL	major hepatectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to evaluate the role of desferrioxamine in the prevention of pancreatic injury following major hepatectomy .
	manualset3
140866	1	408648	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to investigate the effect of vitamin E on the endometrial angiogenic activity and to assess the efficacy of vitamin E supplementation in treating endometrial bleeding in Norplant users .
	manualset3
140867	2	408648	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to investigate the effect of vitamin E on the endometrial angiogenic activity and to assess the efficacy of vitamin E supplementation in treating endometrial bleeding in Norplant users .
	manualset3
140868	3	408648	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to investigate the effect of vitamin E on the endometrial angiogenic activity and to assess the efficacy of vitamin E supplementation in treating endometrial bleeding in Norplant users .
	manualset3
140869	4	408648	5	NULL	NULL	0	NULL	vitamin E	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to investigate the effect of vitamin E on the endometrial angiogenic activity and to assess the efficacy of vitamin E supplementation in treating endometrial bleeding in Norplant users .
	manualset3
140870	5	408648	5	NULL	NULL	0	NULL	endometrial angiogenic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to investigate the effect of vitamin E on the endometrial angiogenic activity and to assess the efficacy of vitamin E supplementation in treating endometrial bleeding in Norplant users .
	manualset3
140871	6	408648	5	NULL	NULL	0	NULL	efficacy 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to investigate the effect of vitamin E on the endometrial angiogenic activity and to assess the efficacy of vitamin E supplementation in treating endometrial bleeding in Norplant users .
	manualset3
140872	7	408648	5	NULL	NULL	0	NULL	vitamin E supplementation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to investigate the effect of vitamin E on the endometrial angiogenic activity and to assess the efficacy of vitamin E supplementation in treating endometrial bleeding in Norplant users .
	manualset3
140873	8	408648	5	NULL	NULL	0	NULL	endometrial bleeding 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to investigate the effect of vitamin E on the endometrial angiogenic activity and to assess the efficacy of vitamin E supplementation in treating endometrial bleeding in Norplant users .
	manualset3
140874	9	408648	5	NULL	NULL	0	NULL	Norplant users	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study is to investigate the effect of vitamin E on the endometrial angiogenic activity and to assess the efficacy of vitamin E supplementation in treating endometrial bleeding in Norplant users .
	manualset3
140875	1	408649	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was first to evaluate NNA prevalence in a French retrospective multicentric series of 210 patients without inhibitors , then to determine their epitope specificity ( against the heavy chain ( HC ) or the light chain ( LC ) of FVIII ) and particularly to assess the prevalence of anti-B domain NNA using specifically designed x-MAP assays .
	manualset3
140876	2	408649	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was first to evaluate NNA prevalence in a French retrospective multicentric series of 210 patients without inhibitors , then to determine their epitope specificity ( against the heavy chain ( HC ) or the light chain ( LC ) of FVIII ) and particularly to assess the prevalence of anti-B domain NNA using specifically designed x-MAP assays .
	manualset3
140877	3	408649	5	NULL	NULL	0	NULL	NNA prevalence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was first to evaluate NNA prevalence in a French retrospective multicentric series of 210 patients without inhibitors , then to determine their epitope specificity ( against the heavy chain ( HC ) or the light chain ( LC ) of FVIII ) and particularly to assess the prevalence of anti-B domain NNA using specifically designed x-MAP assays .
	manualset3
140878	4	408649	5	NULL	NULL	0	NULL	French retrospective multicentric series	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was first to evaluate NNA prevalence in a French retrospective multicentric series of 210 patients without inhibitors , then to determine their epitope specificity ( against the heavy chain ( HC ) or the light chain ( LC ) of FVIII ) and particularly to assess the prevalence of anti-B domain NNA using specifically designed x-MAP assays .
	manualset3
140879	5	408649	5	NULL	NULL	0	NULL	210	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was first to evaluate NNA prevalence in a French retrospective multicentric series of 210 patients without inhibitors , then to determine their epitope specificity ( against the heavy chain ( HC ) or the light chain ( LC ) of FVIII ) and particularly to assess the prevalence of anti-B domain NNA using specifically designed x-MAP assays .
	manualset3
140880	6	408649	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was first to evaluate NNA prevalence in a French retrospective multicentric series of 210 patients without inhibitors , then to determine their epitope specificity ( against the heavy chain ( HC ) or the light chain ( LC ) of FVIII ) and particularly to assess the prevalence of anti-B domain NNA using specifically designed x-MAP assays .
	manualset3
140881	7	408649	5	NULL	NULL	0	NULL	inhibitors 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was first to evaluate NNA prevalence in a French retrospective multicentric series of 210 patients without inhibitors , then to determine their epitope specificity ( against the heavy chain ( HC ) or the light chain ( LC ) of FVIII ) and particularly to assess the prevalence of anti-B domain NNA using specifically designed x-MAP assays .
	manualset3
140882	8	408649	5	NULL	NULL	0	NULL	epitope specificity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was first to evaluate NNA prevalence in a French retrospective multicentric series of 210 patients without inhibitors , then to determine their epitope specificity ( against the heavy chain ( HC ) or the light chain ( LC ) of FVIII ) and particularly to assess the prevalence of anti-B domain NNA using specifically designed x-MAP assays .
	manualset3
140883	9	408649	5	NULL	NULL	0	NULL	heavy chain ( HC )	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was first to evaluate NNA prevalence in a French retrospective multicentric series of 210 patients without inhibitors , then to determine their epitope specificity ( against the heavy chain ( HC ) or the light chain ( LC ) of FVIII ) and particularly to assess the prevalence of anti-B domain NNA using specifically designed x-MAP assays .
	manualset3
140884	10	408649	5	NULL	NULL	0	NULL	light chain ( LC )	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was first to evaluate NNA prevalence in a French retrospective multicentric series of 210 patients without inhibitors , then to determine their epitope specificity ( against the heavy chain ( HC ) or the light chain ( LC ) of FVIII ) and particularly to assess the prevalence of anti-B domain NNA using specifically designed x-MAP assays .
	manualset3
140885	11	408649	5	NULL	NULL	0	NULL	FVIII	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was first to evaluate NNA prevalence in a French retrospective multicentric series of 210 patients without inhibitors , then to determine their epitope specificity ( against the heavy chain ( HC ) or the light chain ( LC ) of FVIII ) and particularly to assess the prevalence of anti-B domain NNA using specifically designed x-MAP assays .
	manualset3
140886	12	408649	5	NULL	NULL	0	NULL	prevalence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was first to evaluate NNA prevalence in a French retrospective multicentric series of 210 patients without inhibitors , then to determine their epitope specificity ( against the heavy chain ( HC ) or the light chain ( LC ) of FVIII ) and particularly to assess the prevalence of anti-B domain NNA using specifically designed x-MAP assays .
	manualset3
140887	13	408649	5	NULL	NULL	0	NULL	anti-B domain NNA	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was first to evaluate NNA prevalence in a French retrospective multicentric series of 210 patients without inhibitors , then to determine their epitope specificity ( against the heavy chain ( HC ) or the light chain ( LC ) of FVIII ) and particularly to assess the prevalence of anti-B domain NNA using specifically designed x-MAP assays .
	manualset3
140888	14	408649	5	NULL	NULL	0	NULL	x-MAP assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was first to evaluate NNA prevalence in a French retrospective multicentric series of 210 patients without inhibitors , then to determine their epitope specificity ( against the heavy chain ( HC ) or the light chain ( LC ) of FVIII ) and particularly to assess the prevalence of anti-B domain NNA using specifically designed x-MAP assays .
	manualset3
140889	1	408650	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to assess the clinical effectiveness of atrioventricular pacing according to the etiology of LVSD , by comparing the outcome of patients with and without coronary artery disease .
	manualset3
140890	2	408650	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to assess the clinical effectiveness of atrioventricular pacing according to the etiology of LVSD , by comparing the outcome of patients with and without coronary artery disease .
	manualset3
140891	3	408650	5	NULL	NULL	0	NULL	clinical effectiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to assess the clinical effectiveness of atrioventricular pacing according to the etiology of LVSD , by comparing the outcome of patients with and without coronary artery disease .
	manualset3
140892	4	408650	5	NULL	NULL	0	NULL	atrioventricular pacing 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to assess the clinical effectiveness of atrioventricular pacing according to the etiology of LVSD , by comparing the outcome of patients with and without coronary artery disease .
	manualset3
140893	5	408650	5	NULL	NULL	NULL	NULL	etiology 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The aim of this study was to assess the clinical effectiveness of atrioventricular pacing according to the etiology of LVSD , by comparing the outcome of patients with and without coronary artery disease .
	manualset3
140894	6	408650	5	NULL	NULL	NULL	NULL	LVSD 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The aim of this study was to assess the clinical effectiveness of atrioventricular pacing according to the etiology of LVSD , by comparing the outcome of patients with and without coronary artery disease .
	manualset3
140895	7	408650	5	NULL	NULL	0	NULL	outcome 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to assess the clinical effectiveness of atrioventricular pacing according to the etiology of LVSD , by comparing the outcome of patients with and without coronary artery disease .
	manualset3
140896	8	408650	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to assess the clinical effectiveness of atrioventricular pacing according to the etiology of LVSD , by comparing the outcome of patients with and without coronary artery disease .
	manualset3
140897	9	408650	5	NULL	NULL	0	NULL	coronary artery disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to assess the clinical effectiveness of atrioventricular pacing according to the etiology of LVSD , by comparing the outcome of patients with and without coronary artery disease .
	manualset3
140898	1	408651	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to assess the effect of chronic administration of NCX4016 ( 2 acetoxy-benzoate 2 - ( 2-nitroxymethyl ) - phenyl ester ) , a nitric oxide-releasing aspirin derivative on the consequences of coronary artery occlusion in streptozotocin-diabetic rats .
	manualset3
140899	2	408651	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to assess the effect of chronic administration of NCX4016 ( 2 acetoxy-benzoate 2 - ( 2-nitroxymethyl ) - phenyl ester ) , a nitric oxide-releasing aspirin derivative on the consequences of coronary artery occlusion in streptozotocin-diabetic rats .
	manualset3
140900	3	408651	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to assess the effect of chronic administration of NCX4016 ( 2 acetoxy-benzoate 2 - ( 2-nitroxymethyl ) - phenyl ester ) , a nitric oxide-releasing aspirin derivative on the consequences of coronary artery occlusion in streptozotocin-diabetic rats .
	manualset3
140901	4	408651	5	NULL	NULL	0	NULL	 chronic administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to assess the effect of chronic administration of NCX4016 ( 2 acetoxy-benzoate 2 - ( 2-nitroxymethyl ) - phenyl ester ) , a nitric oxide-releasing aspirin derivative on the consequences of coronary artery occlusion in streptozotocin-diabetic rats .
	manualset3
140902	5	408651	5	NULL	NULL	0	NULL	NCX4016 ( 2 acetoxy-benzoate 2 - ( 2-nitroxymethyl ) - phenyl ester ) , a nitric oxide-releasing aspirin derivative	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to assess the effect of chronic administration of NCX4016 ( 2 acetoxy-benzoate 2 - ( 2-nitroxymethyl ) - phenyl ester ) , a nitric oxide-releasing aspirin derivative on the consequences of coronary artery occlusion in streptozotocin-diabetic rats .
	manualset3
140903	6	408651	5	NULL	NULL	0	NULL	consequences 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to assess the effect of chronic administration of NCX4016 ( 2 acetoxy-benzoate 2 - ( 2-nitroxymethyl ) - phenyl ester ) , a nitric oxide-releasing aspirin derivative on the consequences of coronary artery occlusion in streptozotocin-diabetic rats .
	manualset3
140904	7	408651	5	NULL	NULL	0	NULL	coronary artery occlusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to assess the effect of chronic administration of NCX4016 ( 2 acetoxy-benzoate 2 - ( 2-nitroxymethyl ) - phenyl ester ) , a nitric oxide-releasing aspirin derivative on the consequences of coronary artery occlusion in streptozotocin-diabetic rats .
	manualset3
140905	8	408651	5	NULL	NULL	0	NULL	streptozotocin-diabetic rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to assess the effect of chronic administration of NCX4016 ( 2 acetoxy-benzoate 2 - ( 2-nitroxymethyl ) - phenyl ester ) , a nitric oxide-releasing aspirin derivative on the consequences of coronary artery occlusion in streptozotocin-diabetic rats .
	manualset3
140906	1	408652	5	NULL	NULL	0	NULL	review 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of 9 studies gave evidence that gays ' children were ( a ) more apt to adopt homosexual interests and activities , ( b ) more apt to report sexual confusion , ( c ) more apt to be socially disturbed , ( d ) more apt to abuse substances , ( e ) less apt to get married , ( f ) more apt to have difficulty in attachment and loving relationships , ( g ) less religious and more unconventionally religious , ( h ) more apt to have emotional difficulties , ( i ) more frequently exposed to parental molestation , and ( j ) prone to more frequent sexual acting out .
	manualset3
140907	2	408652	5	NULL	NULL	0	NULL	9 studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of 9 studies gave evidence that gays ' children were ( a ) more apt to adopt homosexual interests and activities , ( b ) more apt to report sexual confusion , ( c ) more apt to be socially disturbed , ( d ) more apt to abuse substances , ( e ) less apt to get married , ( f ) more apt to have difficulty in attachment and loving relationships , ( g ) less religious and more unconventionally religious , ( h ) more apt to have emotional difficulties , ( i ) more frequently exposed to parental molestation , and ( j ) prone to more frequent sexual acting out .
	manualset3
140908	3	408652	5	NULL	NULL	0	NULL	 gays ' children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of 9 studies gave evidence that gays ' children were ( a ) more apt to adopt homosexual interests and activities , ( b ) more apt to report sexual confusion , ( c ) more apt to be socially disturbed , ( d ) more apt to abuse substances , ( e ) less apt to get married , ( f ) more apt to have difficulty in attachment and loving relationships , ( g ) less religious and more unconventionally religious , ( h ) more apt to have emotional difficulties , ( i ) more frequently exposed to parental molestation , and ( j ) prone to more frequent sexual acting out .
	manualset3
140909	4	408652	5	NULL	NULL	0	NULL	homosexual interests	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of 9 studies gave evidence that gays ' children were ( a ) more apt to adopt homosexual interests and activities , ( b ) more apt to report sexual confusion , ( c ) more apt to be socially disturbed , ( d ) more apt to abuse substances , ( e ) less apt to get married , ( f ) more apt to have difficulty in attachment and loving relationships , ( g ) less religious and more unconventionally religious , ( h ) more apt to have emotional difficulties , ( i ) more frequently exposed to parental molestation , and ( j ) prone to more frequent sexual acting out .
	manualset3
140910	5	408652	5	NULL	NULL	0	NULL	activities 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of 9 studies gave evidence that gays ' children were ( a ) more apt to adopt homosexual interests and activities , ( b ) more apt to report sexual confusion , ( c ) more apt to be socially disturbed , ( d ) more apt to abuse substances , ( e ) less apt to get married , ( f ) more apt to have difficulty in attachment and loving relationships , ( g ) less religious and more unconventionally religious , ( h ) more apt to have emotional difficulties , ( i ) more frequently exposed to parental molestation , and ( j ) prone to more frequent sexual acting out .
	manualset3
140911	6	408652	5	NULL	NULL	0	NULL	sexual confusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of 9 studies gave evidence that gays ' children were ( a ) more apt to adopt homosexual interests and activities , ( b ) more apt to report sexual confusion , ( c ) more apt to be socially disturbed , ( d ) more apt to abuse substances , ( e ) less apt to get married , ( f ) more apt to have difficulty in attachment and loving relationships , ( g ) less religious and more unconventionally religious , ( h ) more apt to have emotional difficulties , ( i ) more frequently exposed to parental molestation , and ( j ) prone to more frequent sexual acting out .
	manualset3
140912	7	408652	5	NULL	NULL	0	NULL	difficulty in attachment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of 9 studies gave evidence that gays ' children were ( a ) more apt to adopt homosexual interests and activities , ( b ) more apt to report sexual confusion , ( c ) more apt to be socially disturbed , ( d ) more apt to abuse substances , ( e ) less apt to get married , ( f ) more apt to have difficulty in attachment and loving relationships , ( g ) less religious and more unconventionally religious , ( h ) more apt to have emotional difficulties , ( i ) more frequently exposed to parental molestation , and ( j ) prone to more frequent sexual acting out .
	manualset3
140913	8	408652	5	NULL	NULL	0	NULL	relationships 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of 9 studies gave evidence that gays ' children were ( a ) more apt to adopt homosexual interests and activities , ( b ) more apt to report sexual confusion , ( c ) more apt to be socially disturbed , ( d ) more apt to abuse substances , ( e ) less apt to get married , ( f ) more apt to have difficulty in attachment and loving relationships , ( g ) less religious and more unconventionally religious , ( h ) more apt to have emotional difficulties , ( i ) more frequently exposed to parental molestation , and ( j ) prone to more frequent sexual acting out .
	manualset3
140914	9	408652	5	NULL	NULL	0	NULL	emotional difficulties	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of 9 studies gave evidence that gays ' children were ( a ) more apt to adopt homosexual interests and activities , ( b ) more apt to report sexual confusion , ( c ) more apt to be socially disturbed , ( d ) more apt to abuse substances , ( e ) less apt to get married , ( f ) more apt to have difficulty in attachment and loving relationships , ( g ) less religious and more unconventionally religious , ( h ) more apt to have emotional difficulties , ( i ) more frequently exposed to parental molestation , and ( j ) prone to more frequent sexual acting out .
	manualset3
140915	10	408652	5	NULL	NULL	0	NULL	parental molestation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of 9 studies gave evidence that gays ' children were ( a ) more apt to adopt homosexual interests and activities , ( b ) more apt to report sexual confusion , ( c ) more apt to be socially disturbed , ( d ) more apt to abuse substances , ( e ) less apt to get married , ( f ) more apt to have difficulty in attachment and loving relationships , ( g ) less religious and more unconventionally religious , ( h ) more apt to have emotional difficulties , ( i ) more frequently exposed to parental molestation , and ( j ) prone to more frequent sexual acting out .
	manualset3
140916	11	408652	5	NULL	NULL	0	NULL	sexual acting out	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of 9 studies gave evidence that gays ' children were ( a ) more apt to adopt homosexual interests and activities , ( b ) more apt to report sexual confusion , ( c ) more apt to be socially disturbed , ( d ) more apt to abuse substances , ( e ) less apt to get married , ( f ) more apt to have difficulty in attachment and loving relationships , ( g ) less religious and more unconventionally religious , ( h ) more apt to have emotional difficulties , ( i ) more frequently exposed to parental molestation , and ( j ) prone to more frequent sexual acting out .
	manualset3
144837	12	408652	5	NULL	NULL	0	NULL	substances 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of 9 studies gave evidence that gays ' children were ( a ) more apt to adopt homosexual interests and activities , ( b ) more apt to report sexual confusion , ( c ) more apt to be socially disturbed , ( d ) more apt to abuse substances , ( e ) less apt to get married , ( f ) more apt to have difficulty in attachment and loving relationships , ( g ) less religious and more unconventionally religious , ( h ) more apt to have emotional difficulties , ( i ) more frequently exposed to parental molestation , and ( j ) prone to more frequent sexual acting out .
	manualset3
140917	1	408653	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to assess the possible mediation of endogenous opioids in the effects of gonadal hormones on the responses to formalin pain .
	manualset3
140918	2	408653	5	NULL	NULL	0	NULL	study 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to assess the possible mediation of endogenous opioids in the effects of gonadal hormones on the responses to formalin pain .
	manualset3
140919	3	408653	5	NULL	NULL	0	NULL	mediation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to assess the possible mediation of endogenous opioids in the effects of gonadal hormones on the responses to formalin pain .
	manualset3
140920	4	408653	5	NULL	NULL	0	NULL	endogenous opioids 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to assess the possible mediation of endogenous opioids in the effects of gonadal hormones on the responses to formalin pain .
	manualset3
140921	5	408653	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to assess the possible mediation of endogenous opioids in the effects of gonadal hormones on the responses to formalin pain .
	manualset3
140922	6	408653	5	NULL	NULL	0	NULL	gonadal hormones	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to assess the possible mediation of endogenous opioids in the effects of gonadal hormones on the responses to formalin pain .
	manualset3
140923	7	408653	5	NULL	NULL	0	NULL	responses 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to assess the possible mediation of endogenous opioids in the effects of gonadal hormones on the responses to formalin pain .
	manualset3
140924	8	408653	5	NULL	NULL	0	NULL	formalin pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to assess the possible mediation of endogenous opioids in the effects of gonadal hormones on the responses to formalin pain .
	manualset3
140925	1	408654	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to carry out a comparative analysis of nutritional status and inflammatory response in CRC patients with or without intestinal obstruction .
	manualset3
140926	2	408654	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to carry out a comparative analysis of nutritional status and inflammatory response in CRC patients with or without intestinal obstruction .
	manualset3
140927	3	408654	5	NULL	NULL	0	NULL	comparative analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to carry out a comparative analysis of nutritional status and inflammatory response in CRC patients with or without intestinal obstruction .
	manualset3
140928	4	408654	5	NULL	NULL	0	NULL	nutritional status	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to carry out a comparative analysis of nutritional status and inflammatory response in CRC patients with or without intestinal obstruction .
	manualset3
140929	5	408654	5	NULL	NULL	0	NULL	inflammatory response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to carry out a comparative analysis of nutritional status and inflammatory response in CRC patients with or without intestinal obstruction .
	manualset3
140930	6	408654	5	NULL	NULL	0	NULL	 CRC patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to carry out a comparative analysis of nutritional status and inflammatory response in CRC patients with or without intestinal obstruction .
	manualset3
140931	7	408654	5	NULL	NULL	0	NULL	intestinal obstruction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to carry out a comparative analysis of nutritional status and inflammatory response in CRC patients with or without intestinal obstruction .
	manualset3
140932	1	408655	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to describe a larger number of medication errors with respect to harm , involved medicines and involved system problems - thus providing information for the development of IT-based decision support .
	manualset3
140933	2	408655	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to describe a larger number of medication errors with respect to harm , involved medicines and involved system problems - thus providing information for the development of IT-based decision support .
	manualset3
140934	3	408655	5	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to describe a larger number of medication errors with respect to harm , involved medicines and involved system problems - thus providing information for the development of IT-based decision support .
	manualset3
140935	4	408655	5	NULL	NULL	0	NULL	medication errors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to describe a larger number of medication errors with respect to harm , involved medicines and involved system problems - thus providing information for the development of IT-based decision support .
	manualset3
140936	5	408655	5	NULL	NULL	0	NULL	medicines 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to describe a larger number of medication errors with respect to harm , involved medicines and involved system problems - thus providing information for the development of IT-based decision support .
	manualset3
140937	6	408655	5	NULL	NULL	NULL	NULL	system problems	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The aim of this study was to describe a larger number of medication errors with respect to harm , involved medicines and involved system problems - thus providing information for the development of IT-based decision support .
	manualset3
140938	7	408655	5	NULL	NULL	0	NULL	information 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to describe a larger number of medication errors with respect to harm , involved medicines and involved system problems - thus providing information for the development of IT-based decision support .
	manualset3
140939	8	408655	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to describe a larger number of medication errors with respect to harm , involved medicines and involved system problems - thus providing information for the development of IT-based decision support .
	manualset3
140940	9	408655	5	NULL	NULL	0	NULL	IT-based decision support	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to describe a larger number of medication errors with respect to harm , involved medicines and involved system problems - thus providing information for the development of IT-based decision support .
	manualset3
140941	1	408656	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to describe psychiatric nurses ' experiences of participating in reflection groups focused on the use of coercion , in relation to their views regarding systematic clinical supervision and staff support .
	manualset3
140942	2	408656	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to describe psychiatric nurses ' experiences of participating in reflection groups focused on the use of coercion , in relation to their views regarding systematic clinical supervision and staff support .
	manualset3
140943	3	408656	5	NULL	NULL	0	NULL	psychiatric nurses ' experiences 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to describe psychiatric nurses ' experiences of participating in reflection groups focused on the use of coercion , in relation to their views regarding systematic clinical supervision and staff support .
	manualset3
140944	4	408656	5	NULL	NULL	0	NULL	reflection groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to describe psychiatric nurses ' experiences of participating in reflection groups focused on the use of coercion , in relation to their views regarding systematic clinical supervision and staff support .
	manualset3
140945	5	408656	5	NULL	NULL	0	NULL	coercion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to describe psychiatric nurses ' experiences of participating in reflection groups focused on the use of coercion , in relation to their views regarding systematic clinical supervision and staff support .
	manualset3
140946	6	408656	5	NULL	NULL	0	NULL	relation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to describe psychiatric nurses ' experiences of participating in reflection groups focused on the use of coercion , in relation to their views regarding systematic clinical supervision and staff support .
	manualset3
140947	7	408656	5	NULL	NULL	0	NULL	views 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to describe psychiatric nurses ' experiences of participating in reflection groups focused on the use of coercion , in relation to their views regarding systematic clinical supervision and staff support .
	manualset3
140948	8	408656	5	NULL	NULL	0	NULL	systematic clinical supervision	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to describe psychiatric nurses ' experiences of participating in reflection groups focused on the use of coercion , in relation to their views regarding systematic clinical supervision and staff support .
	manualset3
140949	9	408656	5	NULL	NULL	0	NULL	staff support	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to describe psychiatric nurses ' experiences of participating in reflection groups focused on the use of coercion , in relation to their views regarding systematic clinical supervision and staff support .
	manualset3
140950	1	408657	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to determine whether Rb2 , a type of ginsenoside , regulates hepatic gluconeogenesis through AMP-activated protein kinase ( AMPK ) and the orphan nuclear receptor small heterodimer partner ( SHP ) in hyperlipidemic conditions used as an in vitro model of type 2 diabetes .
	manualset3
140951	2	408657	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to determine whether Rb2 , a type of ginsenoside , regulates hepatic gluconeogenesis through AMP-activated protein kinase ( AMPK ) and the orphan nuclear receptor small heterodimer partner ( SHP ) in hyperlipidemic conditions used as an in vitro model of type 2 diabetes .
	manualset3
140952	3	408657	5	NULL	NULL	0	NULL	Rb2 , a type of ginsenoside 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to determine whether Rb2 , a type of ginsenoside , regulates hepatic gluconeogenesis through AMP-activated protein kinase ( AMPK ) and the orphan nuclear receptor small heterodimer partner ( SHP ) in hyperlipidemic conditions used as an in vitro model of type 2 diabetes .
	manualset3
140953	4	408657	5	NULL	NULL	0	NULL	hepatic gluconeogenesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to determine whether Rb2 , a type of ginsenoside , regulates hepatic gluconeogenesis through AMP-activated protein kinase ( AMPK ) and the orphan nuclear receptor small heterodimer partner ( SHP ) in hyperlipidemic conditions used as an in vitro model of type 2 diabetes .
	manualset3
140954	5	408657	5	NULL	NULL	0	NULL	AMP-activated protein kinase ( AMPK )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to determine whether Rb2 , a type of ginsenoside , regulates hepatic gluconeogenesis through AMP-activated protein kinase ( AMPK ) and the orphan nuclear receptor small heterodimer partner ( SHP ) in hyperlipidemic conditions used as an in vitro model of type 2 diabetes .
	manualset3
140955	6	408657	5	NULL	NULL	0	NULL	orphan nuclear receptor small heterodimer partner ( SHP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to determine whether Rb2 , a type of ginsenoside , regulates hepatic gluconeogenesis through AMP-activated protein kinase ( AMPK ) and the orphan nuclear receptor small heterodimer partner ( SHP ) in hyperlipidemic conditions used as an in vitro model of type 2 diabetes .
	manualset3
140956	7	408657	5	NULL	NULL	0	NULL	hyperlipidemic conditions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to determine whether Rb2 , a type of ginsenoside , regulates hepatic gluconeogenesis through AMP-activated protein kinase ( AMPK ) and the orphan nuclear receptor small heterodimer partner ( SHP ) in hyperlipidemic conditions used as an in vitro model of type 2 diabetes .
	manualset3
140957	8	408657	5	NULL	NULL	0	NULL	 in vitro model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to determine whether Rb2 , a type of ginsenoside , regulates hepatic gluconeogenesis through AMP-activated protein kinase ( AMPK ) and the orphan nuclear receptor small heterodimer partner ( SHP ) in hyperlipidemic conditions used as an in vitro model of type 2 diabetes .
	manualset3
140958	9	408657	5	NULL	NULL	0	NULL	type 2 diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to determine whether Rb2 , a type of ginsenoside , regulates hepatic gluconeogenesis through AMP-activated protein kinase ( AMPK ) and the orphan nuclear receptor small heterodimer partner ( SHP ) in hyperlipidemic conditions used as an in vitro model of type 2 diabetes .
	manualset3
140959	1	408658	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to determine whether rhBMP-2 might improve the outcome of this disorder .
	manualset3
140960	2	408658	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to determine whether rhBMP-2 might improve the outcome of this disorder .
	manualset3
140961	3	408658	5	NULL	NULL	0	NULL	rhBMP-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to determine whether rhBMP-2 might improve the outcome of this disorder .
	manualset3
140962	4	408658	5	NULL	NULL	0	NULL	outcome 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to determine whether rhBMP-2 might improve the outcome of this disorder .
	manualset3
140963	5	408658	5	NULL	NULL	0	NULL	disorder 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to determine whether rhBMP-2 might improve the outcome of this disorder .
	manualset3
140964	1	408659	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to determine whether supplementing the diet with flaxseed could protect against atherosclerosis induced by a diet enriched in TFA .
	manualset3
140965	2	408659	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to determine whether supplementing the diet with flaxseed could protect against atherosclerosis induced by a diet enriched in TFA .
	manualset3
140966	3	408659	5	NULL	NULL	0	NULL	diet 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to determine whether supplementing the diet with flaxseed could protect against atherosclerosis induced by a diet enriched in TFA .
	manualset3
140967	4	408659	5	NULL	NULL	0	NULL	flaxseed 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to determine whether supplementing the diet with flaxseed could protect against atherosclerosis induced by a diet enriched in TFA .
	manualset3
140968	5	408659	5	NULL	NULL	0	NULL	atherosclerosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to determine whether supplementing the diet with flaxseed could protect against atherosclerosis induced by a diet enriched in TFA .
	manualset3
140969	6	408659	5	NULL	NULL	0	NULL	diet 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to determine whether supplementing the diet with flaxseed could protect against atherosclerosis induced by a diet enriched in TFA .
	manualset3
140970	7	408659	5	NULL	NULL	0	NULL	TFA 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to determine whether supplementing the diet with flaxseed could protect against atherosclerosis induced by a diet enriched in TFA .
	manualset3
140971	1	408660	5	NULL	NULL	0	NULL	review 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of domestic and foreign literature concerning cardiac pathology in patients with Churg-Strauss syndrome is presented .
	manualset3
140972	2	408660	5	NULL	NULL	0	NULL	domestic literature 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of domestic and foreign literature concerning cardiac pathology in patients with Churg-Strauss syndrome is presented .
	manualset3
140973	3	408660	5	NULL	NULL	0	NULL	foreign literature 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of domestic and foreign literature concerning cardiac pathology in patients with Churg-Strauss syndrome is presented .
	manualset3
140974	4	408660	5	NULL	NULL	NULL	NULL	cardiac pathology	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A review of domestic and foreign literature concerning cardiac pathology in patients with Churg-Strauss syndrome is presented .
	manualset3
140975	5	408660	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of domestic and foreign literature concerning cardiac pathology in patients with Churg-Strauss syndrome is presented .
	manualset3
140976	6	408660	5	NULL	NULL	0	NULL	Churg-Strauss syndrome 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of domestic and foreign literature concerning cardiac pathology in patients with Churg-Strauss syndrome is presented .
	manualset3
140977	1	408661	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate behavioral changes and mitochondrial dysfunction in rats administered ketamine for 7 consecutive days .
	manualset3
140978	2	408661	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate behavioral changes and mitochondrial dysfunction in rats administered ketamine for 7 consecutive days .
	manualset3
140979	3	408661	5	NULL	NULL	0	NULL	behavioral changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate behavioral changes and mitochondrial dysfunction in rats administered ketamine for 7 consecutive days .
	manualset3
140980	4	408661	5	NULL	NULL	0	NULL	mitochondrial dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate behavioral changes and mitochondrial dysfunction in rats administered ketamine for 7 consecutive days .
	manualset3
140981	5	408661	5	NULL	NULL	0	NULL	rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate behavioral changes and mitochondrial dysfunction in rats administered ketamine for 7 consecutive days .
	manualset3
140982	6	408661	5	NULL	NULL	0	NULL	ketamine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate behavioral changes and mitochondrial dysfunction in rats administered ketamine for 7 consecutive days .
	manualset3
140983	7	408661	5	NULL	NULL	0	NULL	7 consecutive days	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate behavioral changes and mitochondrial dysfunction in rats administered ketamine for 7 consecutive days .
	manualset3
140984	1	408662	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the anthelmintic activity of hexane ( HE ) , ethyl acetate ( EA ) and ethanol ( EE ) extracts obtained from the seeds of Jatropha curcas using the egg hatch inhibition assay ( EHA ) and the artificial larval exsheathment inhibition assay ( LEIA ) .
	manualset3
140985	2	408662	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the anthelmintic activity of hexane ( HE ) , ethyl acetate ( EA ) and ethanol ( EE ) extracts obtained from the seeds of Jatropha curcas using the egg hatch inhibition assay ( EHA ) and the artificial larval exsheathment inhibition assay ( LEIA ) .
	manualset3
140986	3	408662	5	NULL	NULL	0	NULL	anthelmintic activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the anthelmintic activity of hexane ( HE ) , ethyl acetate ( EA ) and ethanol ( EE ) extracts obtained from the seeds of Jatropha curcas using the egg hatch inhibition assay ( EHA ) and the artificial larval exsheathment inhibition assay ( LEIA ) .
	manualset3
140987	4	408662	5	NULL	NULL	0	NULL	hexane ( HE )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the anthelmintic activity of hexane ( HE ) , ethyl acetate ( EA ) and ethanol ( EE ) extracts obtained from the seeds of Jatropha curcas using the egg hatch inhibition assay ( EHA ) and the artificial larval exsheathment inhibition assay ( LEIA ) .
	manualset3
140988	5	408662	5	NULL	NULL	0	NULL	ethyl acetate ( EA )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the anthelmintic activity of hexane ( HE ) , ethyl acetate ( EA ) and ethanol ( EE ) extracts obtained from the seeds of Jatropha curcas using the egg hatch inhibition assay ( EHA ) and the artificial larval exsheathment inhibition assay ( LEIA ) .
	manualset3
140989	6	408662	5	NULL	NULL	0	NULL	ethanol ( EE ) extracts	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the anthelmintic activity of hexane ( HE ) , ethyl acetate ( EA ) and ethanol ( EE ) extracts obtained from the seeds of Jatropha curcas using the egg hatch inhibition assay ( EHA ) and the artificial larval exsheathment inhibition assay ( LEIA ) .
	manualset3
140990	7	408662	5	NULL	NULL	0	NULL	seeds 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the anthelmintic activity of hexane ( HE ) , ethyl acetate ( EA ) and ethanol ( EE ) extracts obtained from the seeds of Jatropha curcas using the egg hatch inhibition assay ( EHA ) and the artificial larval exsheathment inhibition assay ( LEIA ) .
	manualset3
140991	8	408662	5	NULL	NULL	0	NULL	Jatropha curcas	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the anthelmintic activity of hexane ( HE ) , ethyl acetate ( EA ) and ethanol ( EE ) extracts obtained from the seeds of Jatropha curcas using the egg hatch inhibition assay ( EHA ) and the artificial larval exsheathment inhibition assay ( LEIA ) .
	manualset3
140992	9	408662	5	NULL	NULL	0	NULL	egg hatch inhibition assay ( EHA )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the anthelmintic activity of hexane ( HE ) , ethyl acetate ( EA ) and ethanol ( EE ) extracts obtained from the seeds of Jatropha curcas using the egg hatch inhibition assay ( EHA ) and the artificial larval exsheathment inhibition assay ( LEIA ) .
	manualset3
140993	10	408662	5	NULL	NULL	0	NULL	artificial larval exsheathment inhibition assay ( LEIA ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the anthelmintic activity of hexane ( HE ) , ethyl acetate ( EA ) and ethanol ( EE ) extracts obtained from the seeds of Jatropha curcas using the egg hatch inhibition assay ( EHA ) and the artificial larval exsheathment inhibition assay ( LEIA ) .
	manualset3
140994	1	408663	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the pharmacokinetics , pharmacodynamics and anti-tumour efficacy of the first specific inhibitor , an anti-human ADAM17 IgG antibody , clone D1 ( A12 ) .
	manualset3
140995	2	408663	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the pharmacokinetics , pharmacodynamics and anti-tumour efficacy of the first specific inhibitor , an anti-human ADAM17 IgG antibody , clone D1 ( A12 ) .
	manualset3
140996	3	408663	5	NULL	NULL	0	NULL	pharmacokinetics 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the pharmacokinetics , pharmacodynamics and anti-tumour efficacy of the first specific inhibitor , an anti-human ADAM17 IgG antibody , clone D1 ( A12 ) .
	manualset3
140997	4	408663	5	NULL	NULL	0	NULL	pharmacodynamics 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the pharmacokinetics , pharmacodynamics and anti-tumour efficacy of the first specific inhibitor , an anti-human ADAM17 IgG antibody , clone D1 ( A12 ) .
	manualset3
140998	5	408663	5	NULL	NULL	0	NULL	anti-tumour efficacy 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the pharmacokinetics , pharmacodynamics and anti-tumour efficacy of the first specific inhibitor , an anti-human ADAM17 IgG antibody , clone D1 ( A12 ) .
	manualset3
140999	6	408663	5	NULL	NULL	0	NULL	first specific inhibitor	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the pharmacokinetics , pharmacodynamics and anti-tumour efficacy of the first specific inhibitor , an anti-human ADAM17 IgG antibody , clone D1 ( A12 ) .
	manualset3
141000	7	408663	5	NULL	NULL	0	NULL	anti-human ADAM17 IgG antibody , clone D1 ( A12 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the pharmacokinetics , pharmacodynamics and anti-tumour efficacy of the first specific inhibitor , an anti-human ADAM17 IgG antibody , clone D1 ( A12 ) .
	manualset3
141001	1	408664	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the relationship between dermal microdialysis ( DMD ) sampling and the dermatopharmacokinetic method when employed simultaneously for bioequivalence ( BE ) investigations of topical formulations .
	manualset3
141002	2	408664	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the relationship between dermal microdialysis ( DMD ) sampling and the dermatopharmacokinetic method when employed simultaneously for bioequivalence ( BE ) investigations of topical formulations .
	manualset3
141003	3	408664	5	NULL	NULL	0	NULL	relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the relationship between dermal microdialysis ( DMD ) sampling and the dermatopharmacokinetic method when employed simultaneously for bioequivalence ( BE ) investigations of topical formulations .
	manualset3
141004	4	408664	5	NULL	NULL	0	NULL	dermal microdialysis ( DMD ) sampling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the relationship between dermal microdialysis ( DMD ) sampling and the dermatopharmacokinetic method when employed simultaneously for bioequivalence ( BE ) investigations of topical formulations .
	manualset3
141005	5	408664	5	NULL	NULL	0	NULL	dermatopharmacokinetic method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the relationship between dermal microdialysis ( DMD ) sampling and the dermatopharmacokinetic method when employed simultaneously for bioequivalence ( BE ) investigations of topical formulations .
	manualset3
141006	6	408664	5	NULL	NULL	0	NULL	bioequivalence ( BE ) investigations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the relationship between dermal microdialysis ( DMD ) sampling and the dermatopharmacokinetic method when employed simultaneously for bioequivalence ( BE ) investigations of topical formulations .
	manualset3
141007	7	408664	5	NULL	NULL	0	NULL	topical formulations	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the relationship between dermal microdialysis ( DMD ) sampling and the dermatopharmacokinetic method when employed simultaneously for bioequivalence ( BE ) investigations of topical formulations .
	manualset3
141008	1	408665	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the secular trend of VLBW in the city of Porto Alegre , a large city in a developed area in southern Brazil , and the potential determinants of this trend during the 1990s and early 2000s .
	manualset3
141009	2	408665	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the secular trend of VLBW in the city of Porto Alegre , a large city in a developed area in southern Brazil , and the potential determinants of this trend during the 1990s and early 2000s .
	manualset3
141010	3	408665	5	NULL	NULL	0	NULL	secular trend	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the secular trend of VLBW in the city of Porto Alegre , a large city in a developed area in southern Brazil , and the potential determinants of this trend during the 1990s and early 2000s .
	manualset3
141011	4	408665	5	NULL	NULL	0	NULL	VLBW 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the secular trend of VLBW in the city of Porto Alegre , a large city in a developed area in southern Brazil , and the potential determinants of this trend during the 1990s and early 2000s .
	manualset3
141012	5	408665	5	NULL	NULL	0	NULL	city 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the secular trend of VLBW in the city of Porto Alegre , a large city in a developed area in southern Brazil , and the potential determinants of this trend during the 1990s and early 2000s .
	manualset3
141013	6	408665	5	NULL	NULL	0	NULL	Porto Alegre	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the secular trend of VLBW in the city of Porto Alegre , a large city in a developed area in southern Brazil , and the potential determinants of this trend during the 1990s and early 2000s .
	manualset3
141014	7	408665	5	NULL	NULL	0	NULL	large city	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the secular trend of VLBW in the city of Porto Alegre , a large city in a developed area in southern Brazil , and the potential determinants of this trend during the 1990s and early 2000s .
	manualset3
141015	8	408665	5	NULL	NULL	0	NULL	developed area 	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the secular trend of VLBW in the city of Porto Alegre , a large city in a developed area in southern Brazil , and the potential determinants of this trend during the 1990s and early 2000s .
	manualset3
141016	9	408665	5	NULL	NULL	0	NULL	southern Brazil	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the secular trend of VLBW in the city of Porto Alegre , a large city in a developed area in southern Brazil , and the potential determinants of this trend during the 1990s and early 2000s .
	manualset3
141017	10	408665	5	NULL	NULL	0	NULL	potential determinants 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the secular trend of VLBW in the city of Porto Alegre , a large city in a developed area in southern Brazil , and the potential determinants of this trend during the 1990s and early 2000s .
	manualset3
141018	11	408665	5	NULL	NULL	0	NULL	trend 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the secular trend of VLBW in the city of Porto Alegre , a large city in a developed area in southern Brazil , and the potential determinants of this trend during the 1990s and early 2000s .
	manualset3
141019	12	408665	5	NULL	NULL	0	NULL	1990s 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the secular trend of VLBW in the city of Porto Alegre , a large city in a developed area in southern Brazil , and the potential determinants of this trend during the 1990s and early 2000s .
	manualset3
141020	13	408665	5	NULL	NULL	0	NULL	early 2000s 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate the secular trend of VLBW in the city of Porto Alegre , a large city in a developed area in southern Brazil , and the potential determinants of this trend during the 1990s and early 2000s .
	manualset3
141021	1	408666	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate this assay in subjects including patients with SCP with steatorrhea , patients with MCP with no steatorrhea , healthy controls , and diseased controls with nonpancreatic malabsorption .
	manualset3
141022	2	408666	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate this assay in subjects including patients with SCP with steatorrhea , patients with MCP with no steatorrhea , healthy controls , and diseased controls with nonpancreatic malabsorption .
	manualset3
141023	3	408666	5	NULL	NULL	0	NULL	assay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate this assay in subjects including patients with SCP with steatorrhea , patients with MCP with no steatorrhea , healthy controls , and diseased controls with nonpancreatic malabsorption .
	manualset3
141024	4	408666	5	NULL	NULL	0	NULL	subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate this assay in subjects including patients with SCP with steatorrhea , patients with MCP with no steatorrhea , healthy controls , and diseased controls with nonpancreatic malabsorption .
	manualset3
141025	5	408666	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate this assay in subjects including patients with SCP with steatorrhea , patients with MCP with no steatorrhea , healthy controls , and diseased controls with nonpancreatic malabsorption .
	manualset3
141026	6	408666	5	NULL	NULL	0	NULL	SCP 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate this assay in subjects including patients with SCP with steatorrhea , patients with MCP with no steatorrhea , healthy controls , and diseased controls with nonpancreatic malabsorption .
	manualset3
141027	7	408666	5	NULL	NULL	0	NULL	steatorrhea 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate this assay in subjects including patients with SCP with steatorrhea , patients with MCP with no steatorrhea , healthy controls , and diseased controls with nonpancreatic malabsorption .
	manualset3
141028	8	408666	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate this assay in subjects including patients with SCP with steatorrhea , patients with MCP with no steatorrhea , healthy controls , and diseased controls with nonpancreatic malabsorption .
	manualset3
141029	9	408666	5	NULL	NULL	0	NULL	MCP 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate this assay in subjects including patients with SCP with steatorrhea , patients with MCP with no steatorrhea , healthy controls , and diseased controls with nonpancreatic malabsorption .
	manualset3
141030	10	408666	5	NULL	NULL	0	NULL	steatorrhea 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate this assay in subjects including patients with SCP with steatorrhea , patients with MCP with no steatorrhea , healthy controls , and diseased controls with nonpancreatic malabsorption .
	manualset3
141031	11	408666	5	NULL	NULL	0	NULL	healthy controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate this assay in subjects including patients with SCP with steatorrhea , patients with MCP with no steatorrhea , healthy controls , and diseased controls with nonpancreatic malabsorption .
	manualset3
141032	12	408666	5	NULL	NULL	0	NULL	diseased controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate this assay in subjects including patients with SCP with steatorrhea , patients with MCP with no steatorrhea , healthy controls , and diseased controls with nonpancreatic malabsorption .
	manualset3
141033	13	408666	5	NULL	NULL	0	NULL	nonpancreatic malabsorption	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate this assay in subjects including patients with SCP with steatorrhea , patients with MCP with no steatorrhea , healthy controls , and diseased controls with nonpancreatic malabsorption .
	manualset3
141034	1	408667	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate whether the implantation of ( 32 ) P radioactive stents with a higher activity level ( 12 to 21 microCi ) combined with a nonaggressive stent implantation strategy could solve the problem of edge restenosis .
	manualset3
141035	2	408667	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate whether the implantation of ( 32 ) P radioactive stents with a higher activity level ( 12 to 21 microCi ) combined with a nonaggressive stent implantation strategy could solve the problem of edge restenosis .
	manualset3
141036	3	408667	5	NULL	NULL	0	NULL	implantation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate whether the implantation of ( 32 ) P radioactive stents with a higher activity level ( 12 to 21 microCi ) combined with a nonaggressive stent implantation strategy could solve the problem of edge restenosis .
	manualset3
141037	4	408667	5	NULL	NULL	0	NULL	 ( 32 ) P radioactive stents	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate whether the implantation of ( 32 ) P radioactive stents with a higher activity level ( 12 to 21 microCi ) combined with a nonaggressive stent implantation strategy could solve the problem of edge restenosis .
	manualset3
141038	5	408667	5	NULL	NULL	0	NULL	higher activity level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate whether the implantation of ( 32 ) P radioactive stents with a higher activity level ( 12 to 21 microCi ) combined with a nonaggressive stent implantation strategy could solve the problem of edge restenosis .
	manualset3
141039	6	408667	5	NULL	NULL	0	NULL	12 to 21 microCi	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate whether the implantation of ( 32 ) P radioactive stents with a higher activity level ( 12 to 21 microCi ) combined with a nonaggressive stent implantation strategy could solve the problem of edge restenosis .
	manualset3
141040	7	408667	5	NULL	NULL	0	NULL	nonaggressive stent implantation strategy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate whether the implantation of ( 32 ) P radioactive stents with a higher activity level ( 12 to 21 microCi ) combined with a nonaggressive stent implantation strategy could solve the problem of edge restenosis .
	manualset3
141041	8	408667	5	NULL	NULL	0	NULL	problem 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate whether the implantation of ( 32 ) P radioactive stents with a higher activity level ( 12 to 21 microCi ) combined with a nonaggressive stent implantation strategy could solve the problem of edge restenosis .
	manualset3
141042	9	408667	5	NULL	NULL	0	NULL	edge restenosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to evaluate whether the implantation of ( 32 ) P radioactive stents with a higher activity level ( 12 to 21 microCi ) combined with a nonaggressive stent implantation strategy could solve the problem of edge restenosis .
	manualset3
141043	1	408668	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to examine the characteristics of the non-responders and the reasons for non-response in a survey of respiratory health .
	manualset3
141044	2	408668	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to examine the characteristics of the non-responders and the reasons for non-response in a survey of respiratory health .
	manualset3
141045	3	408668	5	NULL	NULL	0	NULL	characteristics 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to examine the characteristics of the non-responders and the reasons for non-response in a survey of respiratory health .
	manualset3
141046	4	408668	5	NULL	NULL	0	NULL	non-responders 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to examine the characteristics of the non-responders and the reasons for non-response in a survey of respiratory health .
	manualset3
141047	5	408668	5	NULL	NULL	0	NULL	reasons 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to examine the characteristics of the non-responders and the reasons for non-response in a survey of respiratory health .
	manualset3
141048	6	408668	5	NULL	NULL	0	NULL	non-response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to examine the characteristics of the non-responders and the reasons for non-response in a survey of respiratory health .
	manualset3
141049	7	408668	5	NULL	NULL	0	NULL	survey 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to examine the characteristics of the non-responders and the reasons for non-response in a survey of respiratory health .
	manualset3
141050	8	408668	5	NULL	NULL	0	NULL	respiratory health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to examine the characteristics of the non-responders and the reasons for non-response in a survey of respiratory health .
	manualset3
141051	1	408669	5	NULL	NULL	0	NULL	review 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of impressions of the graft materials indicated a decided preference for PTFE grafts .
	manualset3
141052	2	408669	5	NULL	NULL	0	NULL	impressions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of impressions of the graft materials indicated a decided preference for PTFE grafts .
	manualset3
141053	3	408669	5	NULL	NULL	0	NULL	graft materials	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of impressions of the graft materials indicated a decided preference for PTFE grafts .
	manualset3
141054	4	408669	5	NULL	NULL	0	NULL	preference 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of impressions of the graft materials indicated a decided preference for PTFE grafts .
	manualset3
141055	5	408669	5	NULL	NULL	0	NULL	PTFE grafts	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of impressions of the graft materials indicated a decided preference for PTFE grafts .
	manualset3
141056	1	408670	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to examine the effect of cyclooxygenase ( COX ) -2 on bone response after the placement of implants in the femurs of mice .
	manualset3
141057	2	408670	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to examine the effect of cyclooxygenase ( COX ) -2 on bone response after the placement of implants in the femurs of mice .
	manualset3
141058	3	408670	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to examine the effect of cyclooxygenase ( COX ) -2 on bone response after the placement of implants in the femurs of mice .
	manualset3
141059	4	408670	5	NULL	NULL	0	NULL	cyclooxygenase ( COX ) -2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to examine the effect of cyclooxygenase ( COX ) -2 on bone response after the placement of implants in the femurs of mice .
	manualset3
141060	5	408670	5	NULL	NULL	0	NULL	bone response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to examine the effect of cyclooxygenase ( COX ) -2 on bone response after the placement of implants in the femurs of mice .
	manualset3
141061	6	408670	5	NULL	NULL	0	NULL	placement 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to examine the effect of cyclooxygenase ( COX ) -2 on bone response after the placement of implants in the femurs of mice .
	manualset3
141062	7	408670	5	NULL	NULL	0	NULL	implants 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to examine the effect of cyclooxygenase ( COX ) -2 on bone response after the placement of implants in the femurs of mice .
	manualset3
141063	8	408670	5	NULL	NULL	0	NULL	femurs 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to examine the effect of cyclooxygenase ( COX ) -2 on bone response after the placement of implants in the femurs of mice .
	manualset3
141064	9	408670	5	NULL	NULL	0	NULL	mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to examine the effect of cyclooxygenase ( COX ) -2 on bone response after the placement of implants in the femurs of mice .
	manualset3
141065	1	408671	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to find distinctions of the EEG signal in female depression .
	manualset3
141066	2	408671	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to find distinctions of the EEG signal in female depression .
	manualset3
141067	3	408671	5	NULL	NULL	0	NULL	distinctions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to find distinctions of the EEG signal in female depression .
	manualset3
141068	4	408671	5	NULL	NULL	0	NULL	EEG signal	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to find distinctions of the EEG signal in female depression .
	manualset3
141069	5	408671	5	NULL	NULL	0	NULL	female depression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to find distinctions of the EEG signal in female depression .
	manualset3
141070	1	408672	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to investigate the changes in tracheal sounds and airflow dynamics in patients who underwent surgical medialization of a unilaterally paralysed vocal fold .
	manualset3
141071	2	408672	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to investigate the changes in tracheal sounds and airflow dynamics in patients who underwent surgical medialization of a unilaterally paralysed vocal fold .
	manualset3
141072	3	408672	5	NULL	NULL	0	NULL	tracheal sounds	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to investigate the changes in tracheal sounds and airflow dynamics in patients who underwent surgical medialization of a unilaterally paralysed vocal fold .
	manualset3
141073	4	408672	5	NULL	NULL	0	NULL	airflow dynamics	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to investigate the changes in tracheal sounds and airflow dynamics in patients who underwent surgical medialization of a unilaterally paralysed vocal fold .
	manualset3
141074	5	408672	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to investigate the changes in tracheal sounds and airflow dynamics in patients who underwent surgical medialization of a unilaterally paralysed vocal fold .
	manualset3
141075	6	408672	5	NULL	NULL	0	NULL	surgical medialization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to investigate the changes in tracheal sounds and airflow dynamics in patients who underwent surgical medialization of a unilaterally paralysed vocal fold .
	manualset3
141076	7	408672	5	NULL	NULL	NULL	NULL	unilaterally paralysed vocal fold 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The aim of this study was to investigate the changes in tracheal sounds and airflow dynamics in patients who underwent surgical medialization of a unilaterally paralysed vocal fold .
	manualset3
141077	1	408673	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to investigate the possible pathological relation between mechanical stress and hyperpigmentation .
	manualset3
141078	2	408673	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to investigate the possible pathological relation between mechanical stress and hyperpigmentation .
	manualset3
141079	3	408673	5	NULL	NULL	0	NULL	pathological relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to investigate the possible pathological relation between mechanical stress and hyperpigmentation .
	manualset3
141080	4	408673	5	NULL	NULL	0	NULL	mechanical stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to investigate the possible pathological relation between mechanical stress and hyperpigmentation .
	manualset3
141081	5	408673	5	NULL	NULL	0	NULL	hyperpigmentation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to investigate the possible pathological relation between mechanical stress and hyperpigmentation .
	manualset3
141082	1	408674	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to investigate whether multiple doses of the oral and highly selective dipeptidyl peptidase-4 inhibitor linagliptin affect the steady-state pharmacokinetics of the P-glycoprotein substrate digoxin .
	manualset3
141083	2	408674	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to investigate whether multiple doses of the oral and highly selective dipeptidyl peptidase-4 inhibitor linagliptin affect the steady-state pharmacokinetics of the P-glycoprotein substrate digoxin .
	manualset3
141084	3	408674	5	NULL	NULL	0	NULL	multiple doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to investigate whether multiple doses of the oral and highly selective dipeptidyl peptidase-4 inhibitor linagliptin affect the steady-state pharmacokinetics of the P-glycoprotein substrate digoxin .
	manualset3
141085	4	408674	5	NULL	NULL	0	NULL	dipeptidyl peptidase-4 inhibitor linagliptin	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to investigate whether multiple doses of the oral and highly selective dipeptidyl peptidase-4 inhibitor linagliptin affect the steady-state pharmacokinetics of the P-glycoprotein substrate digoxin .
	manualset3
141086	5	408674	5	NULL	NULL	NULL	NULL	steady-state pharmacokinetics	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The aim of this study was to investigate whether multiple doses of the oral and highly selective dipeptidyl peptidase-4 inhibitor linagliptin affect the steady-state pharmacokinetics of the P-glycoprotein substrate digoxin .
	manualset3
141087	6	408674	5	NULL	NULL	0	NULL	P-glycoprotein substrate digoxin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to investigate whether multiple doses of the oral and highly selective dipeptidyl peptidase-4 inhibitor linagliptin affect the steady-state pharmacokinetics of the P-glycoprotein substrate digoxin .
	manualset3
141088	1	408675	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to investigate whether the effects of early life stress augment the sensitivity of the Ang II pathway .
	manualset3
141089	2	408675	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to investigate whether the effects of early life stress augment the sensitivity of the Ang II pathway .
	manualset3
141090	3	408675	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to investigate whether the effects of early life stress augment the sensitivity of the Ang II pathway .
	manualset3
141091	4	408675	5	NULL	NULL	0	NULL	early life stress	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to investigate whether the effects of early life stress augment the sensitivity of the Ang II pathway .
	manualset3
141092	5	408675	5	NULL	NULL	0	NULL	sensitivity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to investigate whether the effects of early life stress augment the sensitivity of the Ang II pathway .
	manualset3
141093	6	408675	5	NULL	NULL	0	NULL	Ang II pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to investigate whether the effects of early life stress augment the sensitivity of the Ang II pathway .
	manualset3
141094	1	408676	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to look at the effect of knee replacement on the employment status of this group of patients .
	manualset3
141095	2	408676	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to look at the effect of knee replacement on the employment status of this group of patients .
	manualset3
141096	3	408676	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to look at the effect of knee replacement on the employment status of this group of patients .
	manualset3
141097	4	408676	5	NULL	NULL	0	NULL	knee replacement 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to look at the effect of knee replacement on the employment status of this group of patients .
	manualset3
141098	5	408676	5	NULL	NULL	0	NULL	employment status	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to look at the effect of knee replacement on the employment status of this group of patients .
	manualset3
141099	6	408676	5	NULL	NULL	0	NULL	group of patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to look at the effect of knee replacement on the employment status of this group of patients .
	manualset3
141100	1	408677	5	NULL	NULL	0	NULL	review 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of the incidence , pathogenesis , diagnostic modalities , and implications of splenic vein occlusion is included .
	manualset3
141101	2	408677	5	NULL	NULL	0	NULL	incidence 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of the incidence , pathogenesis , diagnostic modalities , and implications of splenic vein occlusion is included .
	manualset3
141102	3	408677	5	NULL	NULL	0	NULL	pathogenesis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of the incidence , pathogenesis , diagnostic modalities , and implications of splenic vein occlusion is included .
	manualset3
141103	4	408677	5	NULL	NULL	0	NULL	diagnostic modalities	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of the incidence , pathogenesis , diagnostic modalities , and implications of splenic vein occlusion is included .
	manualset3
141104	5	408677	5	NULL	NULL	0	NULL	implications 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of the incidence , pathogenesis , diagnostic modalities , and implications of splenic vein occlusion is included .
	manualset3
141105	6	408677	5	NULL	NULL	0	NULL	splenic vein occlusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of the incidence , pathogenesis , diagnostic modalities , and implications of splenic vein occlusion is included .
	manualset3
141106	1	408678	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to test the agreement between stress-induced ST-segment elevation and post-exercise QTc changes in infarct leads , in 36 consecutive patients , studied by coronariography , radionuclide ventriculography and thallium-201 scintigraphy , within 3 months of the acute myocardial infarction .
	manualset3
141107	2	408678	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to test the agreement between stress-induced ST-segment elevation and post-exercise QTc changes in infarct leads , in 36 consecutive patients , studied by coronariography , radionuclide ventriculography and thallium-201 scintigraphy , within 3 months of the acute myocardial infarction .
	manualset3
141109	4	408678	5	NULL	NULL	0	NULL	agreement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to test the agreement between stress-induced ST-segment elevation and post-exercise QTc changes in infarct leads , in 36 consecutive patients , studied by coronariography , radionuclide ventriculography and thallium-201 scintigraphy , within 3 months of the acute myocardial infarction .
	manualset3
141110	5	408678	5	NULL	NULL	0	NULL	stress-induced ST-segment elevation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to test the agreement between stress-induced ST-segment elevation and post-exercise QTc changes in infarct leads , in 36 consecutive patients , studied by coronariography , radionuclide ventriculography and thallium-201 scintigraphy , within 3 months of the acute myocardial infarction .
	manualset3
141111	6	408678	5	NULL	NULL	0	NULL	post-exercise QTc changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to test the agreement between stress-induced ST-segment elevation and post-exercise QTc changes in infarct leads , in 36 consecutive patients , studied by coronariography , radionuclide ventriculography and thallium-201 scintigraphy , within 3 months of the acute myocardial infarction .
	manualset3
141112	7	408678	5	NULL	NULL	0	NULL	infarct leads	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to test the agreement between stress-induced ST-segment elevation and post-exercise QTc changes in infarct leads , in 36 consecutive patients , studied by coronariography , radionuclide ventriculography and thallium-201 scintigraphy , within 3 months of the acute myocardial infarction .
	manualset3
141113	8	408678	5	NULL	NULL	0	NULL	36	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to test the agreement between stress-induced ST-segment elevation and post-exercise QTc changes in infarct leads , in 36 consecutive patients , studied by coronariography , radionuclide ventriculography and thallium-201 scintigraphy , within 3 months of the acute myocardial infarction .
	manualset3
141114	9	408678	5	NULL	NULL	0	NULL	consecutive patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to test the agreement between stress-induced ST-segment elevation and post-exercise QTc changes in infarct leads , in 36 consecutive patients , studied by coronariography , radionuclide ventriculography and thallium-201 scintigraphy , within 3 months of the acute myocardial infarction .
	manualset3
141115	10	408678	5	NULL	NULL	0	NULL	coronariography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to test the agreement between stress-induced ST-segment elevation and post-exercise QTc changes in infarct leads , in 36 consecutive patients , studied by coronariography , radionuclide ventriculography and thallium-201 scintigraphy , within 3 months of the acute myocardial infarction .
	manualset3
141116	11	408678	5	NULL	NULL	NULL	NULL	radionuclide ventriculography	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The aim of this study was to test the agreement between stress-induced ST-segment elevation and post-exercise QTc changes in infarct leads , in 36 consecutive patients , studied by coronariography , radionuclide ventriculography and thallium-201 scintigraphy , within 3 months of the acute myocardial infarction .
	manualset3
141117	12	408678	5	NULL	NULL	0	NULL	thallium-201 scintigraphy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to test the agreement between stress-induced ST-segment elevation and post-exercise QTc changes in infarct leads , in 36 consecutive patients , studied by coronariography , radionuclide ventriculography and thallium-201 scintigraphy , within 3 months of the acute myocardial infarction .
	manualset3
141118	13	408678	5	NULL	NULL	0	NULL	 3 months	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to test the agreement between stress-induced ST-segment elevation and post-exercise QTc changes in infarct leads , in 36 consecutive patients , studied by coronariography , radionuclide ventriculography and thallium-201 scintigraphy , within 3 months of the acute myocardial infarction .
	manualset3
141119	14	408678	5	NULL	NULL	0	NULL	acute myocardial infarction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to test the agreement between stress-induced ST-segment elevation and post-exercise QTc changes in infarct leads , in 36 consecutive patients , studied by coronariography , radionuclide ventriculography and thallium-201 scintigraphy , within 3 months of the acute myocardial infarction .
	manualset3
141120	1	408679	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to verify whether the formation in vitro of crystalline macroaggregates , induced by increasing loads of oxalate , is different in normal subjects as opposed to CaOx stone formers , free from urinary metabolic abnormalities .
	manualset3
141121	2	408679	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to verify whether the formation in vitro of crystalline macroaggregates , induced by increasing loads of oxalate , is different in normal subjects as opposed to CaOx stone formers , free from urinary metabolic abnormalities .
	manualset3
141122	3	408679	5	NULL	NULL	0	NULL	formation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to verify whether the formation in vitro of crystalline macroaggregates , induced by increasing loads of oxalate , is different in normal subjects as opposed to CaOx stone formers , free from urinary metabolic abnormalities .
	manualset3
141123	4	408679	5	NULL	NULL	0	NULL	crystalline macroaggregates	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to verify whether the formation in vitro of crystalline macroaggregates , induced by increasing loads of oxalate , is different in normal subjects as opposed to CaOx stone formers , free from urinary metabolic abnormalities .
	manualset3
141124	5	408679	5	NULL	NULL	0	NULL	increasing loads 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to verify whether the formation in vitro of crystalline macroaggregates , induced by increasing loads of oxalate , is different in normal subjects as opposed to CaOx stone formers , free from urinary metabolic abnormalities .
	manualset3
141125	6	408679	5	NULL	NULL	0	NULL	oxalate 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to verify whether the formation in vitro of crystalline macroaggregates , induced by increasing loads of oxalate , is different in normal subjects as opposed to CaOx stone formers , free from urinary metabolic abnormalities .
	manualset3
141126	7	408679	5	NULL	NULL	0	NULL	normal subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to verify whether the formation in vitro of crystalline macroaggregates , induced by increasing loads of oxalate , is different in normal subjects as opposed to CaOx stone formers , free from urinary metabolic abnormalities .
	manualset3
141127	8	408679	5	NULL	NULL	0	NULL	CaOx stone formers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to verify whether the formation in vitro of crystalline macroaggregates , induced by increasing loads of oxalate , is different in normal subjects as opposed to CaOx stone formers , free from urinary metabolic abnormalities .
	manualset3
141128	9	408679	5	NULL	NULL	0	NULL	urinary metabolic abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to verify whether the formation in vitro of crystalline macroaggregates , induced by increasing loads of oxalate , is different in normal subjects as opposed to CaOx stone formers , free from urinary metabolic abnormalities .
	manualset3
141129	1	408680	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to visualize endogenous NPC migration along the RMS with magnetic resonance imaging ( MRI ) in adult healthy mice .
	manualset3
141130	2	408680	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to visualize endogenous NPC migration along the RMS with magnetic resonance imaging ( MRI ) in adult healthy mice .
	manualset3
141131	3	408680	5	NULL	NULL	0	NULL	endogenous NPC migration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to visualize endogenous NPC migration along the RMS with magnetic resonance imaging ( MRI ) in adult healthy mice .
	manualset3
141132	4	408680	5	NULL	NULL	0	NULL	RMS 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to visualize endogenous NPC migration along the RMS with magnetic resonance imaging ( MRI ) in adult healthy mice .
	manualset3
141133	5	408680	5	NULL	NULL	0	NULL	magnetic resonance imaging ( MRI )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to visualize endogenous NPC migration along the RMS with magnetic resonance imaging ( MRI ) in adult healthy mice .
	manualset3
141134	6	408680	5	NULL	NULL	0	NULL	adult healthy mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this study was to visualize endogenous NPC migration along the RMS with magnetic resonance imaging ( MRI ) in adult healthy mice .
	manualset3
141135	1	408681	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this work was to analyze the amino acid conservation in the HCV-E2-PePHD and quasispecies diversity among HCV-HIV-coinfected patients exhibiting sustained virological response , non-response , or partial response with viral relapse to PEG-IFN + RBV by ultra-deep pyrosequencing .
	manualset3
141136	2	408681	5	NULL	NULL	0	NULL	amino acid conservation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this work was to analyze the amino acid conservation in the HCV-E2-PePHD and quasispecies diversity among HCV-HIV-coinfected patients exhibiting sustained virological response , non-response , or partial response with viral relapse to PEG-IFN + RBV by ultra-deep pyrosequencing .
	manualset3
141137	3	408681	5	NULL	NULL	0	NULL	HCV-E2-PePHD	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this work was to analyze the amino acid conservation in the HCV-E2-PePHD and quasispecies diversity among HCV-HIV-coinfected patients exhibiting sustained virological response , non-response , or partial response with viral relapse to PEG-IFN + RBV by ultra-deep pyrosequencing .
	manualset3
141138	4	408681	5	NULL	NULL	0	NULL	quasispecies diversity	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this work was to analyze the amino acid conservation in the HCV-E2-PePHD and quasispecies diversity among HCV-HIV-coinfected patients exhibiting sustained virological response , non-response , or partial response with viral relapse to PEG-IFN + RBV by ultra-deep pyrosequencing .
	manualset3
141139	5	408681	5	NULL	NULL	0	NULL	HCV-HIV-coinfected patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this work was to analyze the amino acid conservation in the HCV-E2-PePHD and quasispecies diversity among HCV-HIV-coinfected patients exhibiting sustained virological response , non-response , or partial response with viral relapse to PEG-IFN + RBV by ultra-deep pyrosequencing .
	manualset3
141140	6	408681	5	NULL	NULL	0	NULL	virological response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this work was to analyze the amino acid conservation in the HCV-E2-PePHD and quasispecies diversity among HCV-HIV-coinfected patients exhibiting sustained virological response , non-response , or partial response with viral relapse to PEG-IFN + RBV by ultra-deep pyrosequencing .
	manualset3
141141	7	408681	5	NULL	NULL	0	NULL	non-response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this work was to analyze the amino acid conservation in the HCV-E2-PePHD and quasispecies diversity among HCV-HIV-coinfected patients exhibiting sustained virological response , non-response , or partial response with viral relapse to PEG-IFN + RBV by ultra-deep pyrosequencing .
	manualset3
141142	8	408681	5	NULL	NULL	0	NULL	partial response 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this work was to analyze the amino acid conservation in the HCV-E2-PePHD and quasispecies diversity among HCV-HIV-coinfected patients exhibiting sustained virological response , non-response , or partial response with viral relapse to PEG-IFN + RBV by ultra-deep pyrosequencing .
	manualset3
141143	9	408681	5	NULL	NULL	0	NULL	viral relapse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this work was to analyze the amino acid conservation in the HCV-E2-PePHD and quasispecies diversity among HCV-HIV-coinfected patients exhibiting sustained virological response , non-response , or partial response with viral relapse to PEG-IFN + RBV by ultra-deep pyrosequencing .
	manualset3
141144	10	408681	5	NULL	NULL	0	NULL	PEG-IFN + RBV 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this work was to analyze the amino acid conservation in the HCV-E2-PePHD and quasispecies diversity among HCV-HIV-coinfected patients exhibiting sustained virological response , non-response , or partial response with viral relapse to PEG-IFN + RBV by ultra-deep pyrosequencing .
	manualset3
141145	11	408681	5	NULL	NULL	0	NULL	ultra-deep pyrosequencing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this work was to analyze the amino acid conservation in the HCV-E2-PePHD and quasispecies diversity among HCV-HIV-coinfected patients exhibiting sustained virological response , non-response , or partial response with viral relapse to PEG-IFN + RBV by ultra-deep pyrosequencing .
	manualset3
144838	12	408681	5	NULL	NULL	0	NULL	work 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this work was to analyze the amino acid conservation in the HCV-E2-PePHD and quasispecies diversity among HCV-HIV-coinfected patients exhibiting sustained virological response , non-response , or partial response with viral relapse to PEG-IFN + RBV by ultra-deep pyrosequencing .
	manualset3
141146	1	408682	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this work was to determine the expression and cellular distribution of syndecan-1 and -2 ( migration molecules ) and E-cadherin and beta-catenin ( adhesion molecules ) in different stages of prostate cancer progression .
	manualset3
141147	2	408682	5	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this work was to determine the expression and cellular distribution of syndecan-1 and -2 ( migration molecules ) and E-cadherin and beta-catenin ( adhesion molecules ) in different stages of prostate cancer progression .
	manualset3
141148	3	408682	5	NULL	NULL	0	NULL	cellular distribution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this work was to determine the expression and cellular distribution of syndecan-1 and -2 ( migration molecules ) and E-cadherin and beta-catenin ( adhesion molecules ) in different stages of prostate cancer progression .
	manualset3
141149	4	408682	5	NULL	NULL	0	NULL	syndecan-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this work was to determine the expression and cellular distribution of syndecan-1 and -2 ( migration molecules ) and E-cadherin and beta-catenin ( adhesion molecules ) in different stages of prostate cancer progression .
	manualset3
141150	5	408682	5	NULL	NULL	0	NULL	syndecan-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this work was to determine the expression and cellular distribution of syndecan-1 and -2 ( migration molecules ) and E-cadherin and beta-catenin ( adhesion molecules ) in different stages of prostate cancer progression .
	manualset3
141151	6	408682	5	NULL	NULL	0	NULL	migration molecules	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this work was to determine the expression and cellular distribution of syndecan-1 and -2 ( migration molecules ) and E-cadherin and beta-catenin ( adhesion molecules ) in different stages of prostate cancer progression .
	manualset3
141152	7	408682	5	NULL	NULL	0	NULL	E-cadherin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this work was to determine the expression and cellular distribution of syndecan-1 and -2 ( migration molecules ) and E-cadherin and beta-catenin ( adhesion molecules ) in different stages of prostate cancer progression .
	manualset3
141153	8	408682	5	NULL	NULL	0	NULL	beta-catenin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this work was to determine the expression and cellular distribution of syndecan-1 and -2 ( migration molecules ) and E-cadherin and beta-catenin ( adhesion molecules ) in different stages of prostate cancer progression .
	manualset3
141154	9	408682	5	NULL	NULL	0	NULL	adhesion molecules	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this work was to determine the expression and cellular distribution of syndecan-1 and -2 ( migration molecules ) and E-cadherin and beta-catenin ( adhesion molecules ) in different stages of prostate cancer progression .
	manualset3
141155	10	408682	5	NULL	NULL	0	NULL	different stages	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this work was to determine the expression and cellular distribution of syndecan-1 and -2 ( migration molecules ) and E-cadherin and beta-catenin ( adhesion molecules ) in different stages of prostate cancer progression .
	manualset3
141156	11	408682	5	NULL	NULL	0	NULL	prostate cancer progression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this work was to determine the expression and cellular distribution of syndecan-1 and -2 ( migration molecules ) and E-cadherin and beta-catenin ( adhesion molecules ) in different stages of prostate cancer progression .
	manualset3
144839	12	408682	5	NULL	NULL	0	NULL	work 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of this work was to determine the expression and cellular distribution of syndecan-1 and -2 ( migration molecules ) and E-cadherin and beta-catenin ( adhesion molecules ) in different stages of prostate cancer progression .
	manualset3
141157	1	408683	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim was to determine the association of tear fluid cytokine levels and post-PRK corneal haze evaluated by in vivo confocal microscopy .
	manualset3
141158	2	408683	5	NULL	NULL	0	NULL	association 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim was to determine the association of tear fluid cytokine levels and post-PRK corneal haze evaluated by in vivo confocal microscopy .
	manualset3
141159	3	408683	5	NULL	NULL	0	NULL	tear fluid cytokine levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim was to determine the association of tear fluid cytokine levels and post-PRK corneal haze evaluated by in vivo confocal microscopy .
	manualset3
141160	4	408683	5	NULL	NULL	0	NULL	post-PRK corneal haze	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim was to determine the association of tear fluid cytokine levels and post-PRK corneal haze evaluated by in vivo confocal microscopy .
	manualset3
141161	5	408683	5	NULL	NULL	0	NULL	 in vivo confocal microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim was to determine the association of tear fluid cytokine levels and post-PRK corneal haze evaluated by in vivo confocal microscopy .
	manualset3
141162	1	408684	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim was to determine whether the clinical features of tachycardias originating from the right ventricular outflow tract in children with an apparently normal heart could predict the presence and the severity of the histopathological substrate .
	manualset3
141163	2	408684	5	NULL	NULL	0	NULL	clinical features	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim was to determine whether the clinical features of tachycardias originating from the right ventricular outflow tract in children with an apparently normal heart could predict the presence and the severity of the histopathological substrate .
	manualset3
141164	3	408684	5	NULL	NULL	0	NULL	tachycardias 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim was to determine whether the clinical features of tachycardias originating from the right ventricular outflow tract in children with an apparently normal heart could predict the presence and the severity of the histopathological substrate .
	manualset3
141165	4	408684	5	NULL	NULL	0	NULL	right ventricular outflow tract 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim was to determine whether the clinical features of tachycardias originating from the right ventricular outflow tract in children with an apparently normal heart could predict the presence and the severity of the histopathological substrate .
	manualset3
141166	5	408684	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim was to determine whether the clinical features of tachycardias originating from the right ventricular outflow tract in children with an apparently normal heart could predict the presence and the severity of the histopathological substrate .
	manualset3
141167	6	408684	5	NULL	NULL	0	NULL	normal heart	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim was to determine whether the clinical features of tachycardias originating from the right ventricular outflow tract in children with an apparently normal heart could predict the presence and the severity of the histopathological substrate .
	manualset3
141168	7	408684	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim was to determine whether the clinical features of tachycardias originating from the right ventricular outflow tract in children with an apparently normal heart could predict the presence and the severity of the histopathological substrate .
	manualset3
141169	8	408684	5	NULL	NULL	0	NULL	severity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim was to determine whether the clinical features of tachycardias originating from the right ventricular outflow tract in children with an apparently normal heart could predict the presence and the severity of the histopathological substrate .
	manualset3
141170	9	408684	5	NULL	NULL	0	NULL	histopathological substrate 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim was to determine whether the clinical features of tachycardias originating from the right ventricular outflow tract in children with an apparently normal heart could predict the presence and the severity of the histopathological substrate .
	manualset3
141171	1	408685	5	NULL	NULL	0	NULL	aims 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were 1 ) to determine the involvement of NO in IL-1beta-induced alterations in protein expression and 2 ) to investigate the effects of chemically generated NO on protein expression by 2D gel electrophoresis of neonatal rat islet samples .
	manualset3
141172	2	408685	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were 1 ) to determine the involvement of NO in IL-1beta-induced alterations in protein expression and 2 ) to investigate the effects of chemically generated NO on protein expression by 2D gel electrophoresis of neonatal rat islet samples .
	manualset3
141173	3	408685	5	NULL	NULL	0	NULL	involvement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were 1 ) to determine the involvement of NO in IL-1beta-induced alterations in protein expression and 2 ) to investigate the effects of chemically generated NO on protein expression by 2D gel electrophoresis of neonatal rat islet samples .
	manualset3
141174	4	408685	5	NULL	NULL	0	NULL	NO 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were 1 ) to determine the involvement of NO in IL-1beta-induced alterations in protein expression and 2 ) to investigate the effects of chemically generated NO on protein expression by 2D gel electrophoresis of neonatal rat islet samples .
	manualset3
141175	5	408685	5	NULL	NULL	0	NULL	IL-1beta-induced alterations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were 1 ) to determine the involvement of NO in IL-1beta-induced alterations in protein expression and 2 ) to investigate the effects of chemically generated NO on protein expression by 2D gel electrophoresis of neonatal rat islet samples .
	manualset3
141176	6	408685	5	NULL	NULL	0	NULL	protein expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were 1 ) to determine the involvement of NO in IL-1beta-induced alterations in protein expression and 2 ) to investigate the effects of chemically generated NO on protein expression by 2D gel electrophoresis of neonatal rat islet samples .
	manualset3
141177	7	408685	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were 1 ) to determine the involvement of NO in IL-1beta-induced alterations in protein expression and 2 ) to investigate the effects of chemically generated NO on protein expression by 2D gel electrophoresis of neonatal rat islet samples .
	manualset3
141178	8	408685	5	NULL	NULL	0	NULL	NO 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were 1 ) to determine the involvement of NO in IL-1beta-induced alterations in protein expression and 2 ) to investigate the effects of chemically generated NO on protein expression by 2D gel electrophoresis of neonatal rat islet samples .
	manualset3
141179	9	408685	5	NULL	NULL	0	NULL	protein expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were 1 ) to determine the involvement of NO in IL-1beta-induced alterations in protein expression and 2 ) to investigate the effects of chemically generated NO on protein expression by 2D gel electrophoresis of neonatal rat islet samples .
	manualset3
141180	10	408685	5	NULL	NULL	0	NULL	2D gel electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were 1 ) to determine the involvement of NO in IL-1beta-induced alterations in protein expression and 2 ) to investigate the effects of chemically generated NO on protein expression by 2D gel electrophoresis of neonatal rat islet samples .
	manualset3
141181	11	408685	5	NULL	NULL	0	NULL	neonatal rat islet samples	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were 1 ) to determine the involvement of NO in IL-1beta-induced alterations in protein expression and 2 ) to investigate the effects of chemically generated NO on protein expression by 2D gel electrophoresis of neonatal rat islet samples .
	manualset3
141182	1	408686	5	NULL	NULL	0	NULL	aims 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to assess the use of Pap smears in Spain in 2009 to identify factors associated with screening adherence ( predictors ) and assess the trend from 2003 to 2009 .
	manualset3
141183	2	408686	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to assess the use of Pap smears in Spain in 2009 to identify factors associated with screening adherence ( predictors ) and assess the trend from 2003 to 2009 .
	manualset3
141184	3	408686	5	NULL	NULL	0	NULL	Pap smears	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to assess the use of Pap smears in Spain in 2009 to identify factors associated with screening adherence ( predictors ) and assess the trend from 2003 to 2009 .
	manualset3
141185	4	408686	5	NULL	NULL	0	NULL	Spain 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to assess the use of Pap smears in Spain in 2009 to identify factors associated with screening adherence ( predictors ) and assess the trend from 2003 to 2009 .
	manualset3
141186	5	408686	5	NULL	NULL	0	NULL	2009 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to assess the use of Pap smears in Spain in 2009 to identify factors associated with screening adherence ( predictors ) and assess the trend from 2003 to 2009 .
	manualset3
141187	6	408686	5	NULL	NULL	0	NULL	factors associated with screening adherence ( predictors ) 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to assess the use of Pap smears in Spain in 2009 to identify factors associated with screening adherence ( predictors ) and assess the trend from 2003 to 2009 .
	manualset3
141188	7	408686	5	NULL	NULL	0	NULL	trend 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to assess the use of Pap smears in Spain in 2009 to identify factors associated with screening adherence ( predictors ) and assess the trend from 2003 to 2009 .
	manualset3
141189	8	408686	5	NULL	NULL	0	NULL	2003 to 2009 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to assess the use of Pap smears in Spain in 2009 to identify factors associated with screening adherence ( predictors ) and assess the trend from 2003 to 2009 .
	manualset3
144840	9	408686	5	NULL	NULL	0	NULL	use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to assess the use of Pap smears in Spain in 2009 to identify factors associated with screening adherence ( predictors ) and assess the trend from 2003 to 2009 .
	manualset3
141190	1	408687	5	NULL	NULL	0	NULL	aims 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to decipher the molecular mechanisms for transcriptional and post-transcriptional regulation expression of KCNQ1 and KCNE1 genes and to shed light on the molecular mechanisms for their spatial heterogeneity of distribution .
	manualset3
141191	2	408687	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to decipher the molecular mechanisms for transcriptional and post-transcriptional regulation expression of KCNQ1 and KCNE1 genes and to shed light on the molecular mechanisms for their spatial heterogeneity of distribution .
	manualset3
141192	3	408687	5	NULL	NULL	0	NULL	molecular mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to decipher the molecular mechanisms for transcriptional and post-transcriptional regulation expression of KCNQ1 and KCNE1 genes and to shed light on the molecular mechanisms for their spatial heterogeneity of distribution .
	manualset3
141193	4	408687	5	NULL	NULL	0	NULL	transcriptional regulation expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to decipher the molecular mechanisms for transcriptional and post-transcriptional regulation expression of KCNQ1 and KCNE1 genes and to shed light on the molecular mechanisms for their spatial heterogeneity of distribution .
	manualset3
141194	5	408687	5	NULL	NULL	0	NULL	post-transcriptional regulation expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to decipher the molecular mechanisms for transcriptional and post-transcriptional regulation expression of KCNQ1 and KCNE1 genes and to shed light on the molecular mechanisms for their spatial heterogeneity of distribution .
	manualset3
141195	6	408687	5	NULL	NULL	0	NULL	KCNQ1 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to decipher the molecular mechanisms for transcriptional and post-transcriptional regulation expression of KCNQ1 and KCNE1 genes and to shed light on the molecular mechanisms for their spatial heterogeneity of distribution .
	manualset3
141196	7	408687	5	NULL	NULL	0	NULL	KCNE1 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to decipher the molecular mechanisms for transcriptional and post-transcriptional regulation expression of KCNQ1 and KCNE1 genes and to shed light on the molecular mechanisms for their spatial heterogeneity of distribution .
	manualset3
141197	8	408687	5	NULL	NULL	0	NULL	molecular mechanisms 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to decipher the molecular mechanisms for transcriptional and post-transcriptional regulation expression of KCNQ1 and KCNE1 genes and to shed light on the molecular mechanisms for their spatial heterogeneity of distribution .
	manualset3
141198	9	408687	5	NULL	NULL	0	NULL	spatial heterogeneity	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to decipher the molecular mechanisms for transcriptional and post-transcriptional regulation expression of KCNQ1 and KCNE1 genes and to shed light on the molecular mechanisms for their spatial heterogeneity of distribution .
	manualset3
141199	10	408687	5	NULL	NULL	0	NULL	distribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to decipher the molecular mechanisms for transcriptional and post-transcriptional regulation expression of KCNQ1 and KCNE1 genes and to shed light on the molecular mechanisms for their spatial heterogeneity of distribution .
	manualset3
141200	1	408688	5	NULL	NULL	0	NULL	review 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of the literature and a comprehensive discussion on alum irrigation as treatment for haematuria is discussed here to create an awareness regarding this treatment option .
	manualset3
141201	2	408688	5	NULL	NULL	0	NULL	literature 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of the literature and a comprehensive discussion on alum irrigation as treatment for haematuria is discussed here to create an awareness regarding this treatment option .
	manualset3
141202	3	408688	5	NULL	NULL	0	NULL	comprehensive discussion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of the literature and a comprehensive discussion on alum irrigation as treatment for haematuria is discussed here to create an awareness regarding this treatment option .
	manualset3
141203	4	408688	5	NULL	NULL	0	NULL	alum irrigation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of the literature and a comprehensive discussion on alum irrigation as treatment for haematuria is discussed here to create an awareness regarding this treatment option .
	manualset3
141204	5	408688	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of the literature and a comprehensive discussion on alum irrigation as treatment for haematuria is discussed here to create an awareness regarding this treatment option .
	manualset3
141205	6	408688	5	NULL	NULL	0	NULL	haematuria 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of the literature and a comprehensive discussion on alum irrigation as treatment for haematuria is discussed here to create an awareness regarding this treatment option .
	manualset3
141206	7	408688	5	NULL	NULL	0	NULL	awareness 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of the literature and a comprehensive discussion on alum irrigation as treatment for haematuria is discussed here to create an awareness regarding this treatment option .
	manualset3
141207	8	408688	5	NULL	NULL	0	NULL	treatment option	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of the literature and a comprehensive discussion on alum irrigation as treatment for haematuria is discussed here to create an awareness regarding this treatment option .
	manualset3
141208	1	408689	5	NULL	NULL	0	NULL	aims 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to evaluate the stability of - lipoic acid and vitamin A palmitate in the presence of vitamin E ( acetate ) and other antioxidants in lipophilic/hydrophilic medium ( O/W emulsions ) at pH 3.0 , 5.0 , and 7.0 .
	manualset3
141209	2	408689	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to evaluate the stability of - lipoic acid and vitamin A palmitate in the presence of vitamin E ( acetate ) and other antioxidants in lipophilic/hydrophilic medium ( O/W emulsions ) at pH 3.0 , 5.0 , and 7.0 .
	manualset3
141210	3	408689	5	NULL	NULL	0	NULL	stability 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to evaluate the stability of - lipoic acid and vitamin A palmitate in the presence of vitamin E ( acetate ) and other antioxidants in lipophilic/hydrophilic medium ( O/W emulsions ) at pH 3.0 , 5.0 , and 7.0 .
	manualset3
141211	4	408689	5	NULL	NULL	0	NULL	lipoic acid	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to evaluate the stability of - lipoic acid and vitamin A palmitate in the presence of vitamin E ( acetate ) and other antioxidants in lipophilic/hydrophilic medium ( O/W emulsions ) at pH 3.0 , 5.0 , and 7.0 .
	manualset3
141212	5	408689	5	NULL	NULL	0	NULL	vitamin A palmitate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to evaluate the stability of - lipoic acid and vitamin A palmitate in the presence of vitamin E ( acetate ) and other antioxidants in lipophilic/hydrophilic medium ( O/W emulsions ) at pH 3.0 , 5.0 , and 7.0 .
	manualset3
141213	6	408689	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to evaluate the stability of - lipoic acid and vitamin A palmitate in the presence of vitamin E ( acetate ) and other antioxidants in lipophilic/hydrophilic medium ( O/W emulsions ) at pH 3.0 , 5.0 , and 7.0 .
	manualset3
141214	7	408689	5	NULL	NULL	0	NULL	vitamin E ( acetate ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to evaluate the stability of - lipoic acid and vitamin A palmitate in the presence of vitamin E ( acetate ) and other antioxidants in lipophilic/hydrophilic medium ( O/W emulsions ) at pH 3.0 , 5.0 , and 7.0 .
	manualset3
141215	8	408689	5	NULL	NULL	0	NULL	antioxidants 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to evaluate the stability of - lipoic acid and vitamin A palmitate in the presence of vitamin E ( acetate ) and other antioxidants in lipophilic/hydrophilic medium ( O/W emulsions ) at pH 3.0 , 5.0 , and 7.0 .
	manualset3
141216	9	408689	5	NULL	NULL	0	NULL	lipophilic/hydrophilic medium ( O/W emulsions )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to evaluate the stability of - lipoic acid and vitamin A palmitate in the presence of vitamin E ( acetate ) and other antioxidants in lipophilic/hydrophilic medium ( O/W emulsions ) at pH 3.0 , 5.0 , and 7.0 .
	manualset3
141217	10	408689	5	NULL	NULL	0	NULL	pH 3.0	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to evaluate the stability of - lipoic acid and vitamin A palmitate in the presence of vitamin E ( acetate ) and other antioxidants in lipophilic/hydrophilic medium ( O/W emulsions ) at pH 3.0 , 5.0 , and 7.0 .
	manualset3
141218	11	408689	5	NULL	NULL	0	NULL	pH 5.0	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to evaluate the stability of - lipoic acid and vitamin A palmitate in the presence of vitamin E ( acetate ) and other antioxidants in lipophilic/hydrophilic medium ( O/W emulsions ) at pH 3.0 , 5.0 , and 7.0 .
	manualset3
141219	12	408689	5	NULL	NULL	0	NULL	pH 7.0	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to evaluate the stability of - lipoic acid and vitamin A palmitate in the presence of vitamin E ( acetate ) and other antioxidants in lipophilic/hydrophilic medium ( O/W emulsions ) at pH 3.0 , 5.0 , and 7.0 .
	manualset3
141220	1	408690	5	NULL	NULL	0	NULL	aims 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to propose a method for the transformation of values of rennet coagulation time ( RCT ) and curd firmness ( a ( 30 ) ) and to predict the noncoagulation ( NC ) probability of milk samples analyzed using different methodologies .
	manualset3
141221	2	408690	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to propose a method for the transformation of values of rennet coagulation time ( RCT ) and curd firmness ( a ( 30 ) ) and to predict the noncoagulation ( NC ) probability of milk samples analyzed using different methodologies .
	manualset3
141222	3	408690	5	NULL	NULL	0	NULL	method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to propose a method for the transformation of values of rennet coagulation time ( RCT ) and curd firmness ( a ( 30 ) ) and to predict the noncoagulation ( NC ) probability of milk samples analyzed using different methodologies .
	manualset3
141223	4	408690	5	NULL	NULL	0	NULL	transformation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to propose a method for the transformation of values of rennet coagulation time ( RCT ) and curd firmness ( a ( 30 ) ) and to predict the noncoagulation ( NC ) probability of milk samples analyzed using different methodologies .
	manualset3
141224	5	408690	5	NULL	NULL	0	NULL	values 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to propose a method for the transformation of values of rennet coagulation time ( RCT ) and curd firmness ( a ( 30 ) ) and to predict the noncoagulation ( NC ) probability of milk samples analyzed using different methodologies .
	manualset3
141225	6	408690	5	NULL	NULL	0	NULL	rennet coagulation time ( RCT )	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to propose a method for the transformation of values of rennet coagulation time ( RCT ) and curd firmness ( a ( 30 ) ) and to predict the noncoagulation ( NC ) probability of milk samples analyzed using different methodologies .
	manualset3
141226	7	408690	5	NULL	NULL	0	NULL	curd firmness ( a ( 30 ) ) 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to propose a method for the transformation of values of rennet coagulation time ( RCT ) and curd firmness ( a ( 30 ) ) and to predict the noncoagulation ( NC ) probability of milk samples analyzed using different methodologies .
	manualset3
141227	8	408690	5	NULL	NULL	0	NULL	noncoagulation ( NC ) probability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to propose a method for the transformation of values of rennet coagulation time ( RCT ) and curd firmness ( a ( 30 ) ) and to predict the noncoagulation ( NC ) probability of milk samples analyzed using different methodologies .
	manualset3
141228	9	408690	5	NULL	NULL	0	NULL	milk samples	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to propose a method for the transformation of values of rennet coagulation time ( RCT ) and curd firmness ( a ( 30 ) ) and to predict the noncoagulation ( NC ) probability of milk samples analyzed using different methodologies .
	manualset3
141229	10	408690	5	NULL	NULL	0	NULL	methodologies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aims of this study were to propose a method for the transformation of values of rennet coagulation time ( RCT ) and curd firmness ( a ( 30 ) ) and to predict the noncoagulation ( NC ) probability of milk samples analyzed using different methodologies .
	manualset3
141230	1	408691	5	NULL	NULL	0	NULL	air pouches 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The air pouches were harvested 2 or 7days after Bzb injection for molecular and histological analyses .
	manualset3
141231	2	408691	5	NULL	NULL	0	NULL	2 or 7days 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The air pouches were harvested 2 or 7days after Bzb injection for molecular and histological analyses .
	manualset3
141232	3	408691	5	NULL	NULL	0	NULL	Bzb injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The air pouches were harvested 2 or 7days after Bzb injection for molecular and histological analyses .
	manualset3
141233	4	408691	5	NULL	NULL	0	NULL	molecular analyses 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The air pouches were harvested 2 or 7days after Bzb injection for molecular and histological analyses .
	manualset3
141234	5	408691	5	NULL	NULL	0	NULL	histological analyses 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The air pouches were harvested 2 or 7days after Bzb injection for molecular and histological analyses .
	manualset3
141235	1	408692	5	NULL	NULL	0	NULL	air supply rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The air supply rate and the primary air distribution along the grate should be adjusted according to the initial moisture content of the waste .
	manualset3
141236	2	408692	5	NULL	NULL	0	NULL	primary air distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The air supply rate and the primary air distribution along the grate should be adjusted according to the initial moisture content of the waste .
	manualset3
141237	3	408692	5	NULL	NULL	0	NULL	grate 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The air supply rate and the primary air distribution along the grate should be adjusted according to the initial moisture content of the waste .
	manualset3
141238	4	408692	5	NULL	NULL	0	NULL	initial moisture content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The air supply rate and the primary air distribution along the grate should be adjusted according to the initial moisture content of the waste .
	manualset3
141239	5	408692	5	NULL	NULL	0	NULL	waste 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The air supply rate and the primary air distribution along the grate should be adjusted according to the initial moisture content of the waste .
	manualset3
141240	1	408693	5	NULL	NULL	0	NULL	airborne bacterial particles number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The airborne bacterial particles number sampled with 6 grades Andersen sampler at Xidan in Beijing from 1987 to 1988 was calibrated by the alive bioparticles calibration formula .
	manualset3
141241	2	408693	5	NULL	NULL	0	NULL	6 grades Andersen sampler 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The airborne bacterial particles number sampled with 6 grades Andersen sampler at Xidan in Beijing from 1987 to 1988 was calibrated by the alive bioparticles calibration formula .
	manualset3
141242	3	408693	5	NULL	NULL	0	NULL	Xidan 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The airborne bacterial particles number sampled with 6 grades Andersen sampler at Xidan in Beijing from 1987 to 1988 was calibrated by the alive bioparticles calibration formula .
	manualset3
141243	4	408693	5	NULL	NULL	0	NULL	Beijing 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The airborne bacterial particles number sampled with 6 grades Andersen sampler at Xidan in Beijing from 1987 to 1988 was calibrated by the alive bioparticles calibration formula .
	manualset3
141244	5	408693	5	NULL	NULL	0	NULL	1987 to 1988	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The airborne bacterial particles number sampled with 6 grades Andersen sampler at Xidan in Beijing from 1987 to 1988 was calibrated by the alive bioparticles calibration formula .
	manualset3
141245	6	408693	5	NULL	NULL	0	NULL	alive bioparticles calibration formula	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The airborne bacterial particles number sampled with 6 grades Andersen sampler at Xidan in Beijing from 1987 to 1988 was calibrated by the alive bioparticles calibration formula .
	manualset3
141246	1	408694	5	NULL	NULL	0	NULL	albumin-binding domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The albumin-binding domain is derived from Streptococcal protein G and has a strong inherent affinity to human serum albumin ( HSA ) .
	manualset3
141247	2	408694	5	NULL	NULL	0	NULL	Streptococcal protein G	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The albumin-binding domain is derived from Streptococcal protein G and has a strong inherent affinity to human serum albumin ( HSA ) .
	manualset3
141248	3	408694	5	NULL	NULL	0	NULL	strong inherent affinity	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The albumin-binding domain is derived from Streptococcal protein G and has a strong inherent affinity to human serum albumin ( HSA ) .
	manualset3
141249	4	408694	5	NULL	NULL	0	NULL	human serum albumin ( HSA ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The albumin-binding domain is derived from Streptococcal protein G and has a strong inherent affinity to human serum albumin ( HSA ) .
	manualset3
141250	1	408695	5	NULL	NULL	0	NULL	albumin secretion rate 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The albumin secretion rate was higher in pyruvate-supplemented than in non-supplemented cultures .
	manualset3
141251	2	408695	5	NULL	NULL	0	NULL	pyruvate-supplemented cultures 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The albumin secretion rate was higher in pyruvate-supplemented than in non-supplemented cultures .
	manualset3
141252	3	408695	5	NULL	NULL	0	NULL	non-supplemented cultures 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The albumin secretion rate was higher in pyruvate-supplemented than in non-supplemented cultures .
	manualset3
141253	1	408696	5	NULL	NULL	0	NULL	aldehyde oximes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The aldehyde oximes formed on the fiber were desorbed and analyzed by gas chromatography-mass spectrometry ( GC-MS ) .
	manualset3
141254	2	408696	5	NULL	NULL	0	NULL	fiber 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aldehyde oximes formed on the fiber were desorbed and analyzed by gas chromatography-mass spectrometry ( GC-MS ) .
	manualset3
141255	3	408696	5	NULL	NULL	0	NULL	gas chromatography-mass spectrometry ( GC-MS )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aldehyde oximes formed on the fiber were desorbed and analyzed by gas chromatography-mass spectrometry ( GC-MS ) .
	manualset3
141256	1	408697	5	NULL	NULL	0	NULL	algorithm 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The algorithm is based on a Trotter decomposition of the quantum-classical propagator , in conjunction with Monte Carlo sampling of quantum transitions , to yield a surface-hopping representation of the dynamics .
	manualset3
141257	2	408697	5	NULL	NULL	0	NULL	Trotter decomposition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The algorithm is based on a Trotter decomposition of the quantum-classical propagator , in conjunction with Monte Carlo sampling of quantum transitions , to yield a surface-hopping representation of the dynamics .
	manualset3
141258	3	408697	5	NULL	NULL	0	NULL	quantum-classical propagator	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The algorithm is based on a Trotter decomposition of the quantum-classical propagator , in conjunction with Monte Carlo sampling of quantum transitions , to yield a surface-hopping representation of the dynamics .
	manualset3
141259	4	408697	5	NULL	NULL	0	NULL	conjunction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The algorithm is based on a Trotter decomposition of the quantum-classical propagator , in conjunction with Monte Carlo sampling of quantum transitions , to yield a surface-hopping representation of the dynamics .
	manualset3
141260	5	408697	5	NULL	NULL	0	NULL	quantum transitions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The algorithm is based on a Trotter decomposition of the quantum-classical propagator , in conjunction with Monte Carlo sampling of quantum transitions , to yield a surface-hopping representation of the dynamics .
	manualset3
141261	6	408697	5	NULL	NULL	0	NULL	surface-hopping representation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The algorithm is based on a Trotter decomposition of the quantum-classical propagator , in conjunction with Monte Carlo sampling of quantum transitions , to yield a surface-hopping representation of the dynamics .
	manualset3
141262	7	408697	5	NULL	NULL	0	NULL	dynamics 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The algorithm is based on a Trotter decomposition of the quantum-classical propagator , in conjunction with Monte Carlo sampling of quantum transitions , to yield a surface-hopping representation of the dynamics .
	manualset3
141263	1	408698	5	NULL	NULL	0	NULL	review 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of the literature on burns and trauma , October 1960 to August 1961 .
	manualset3
141264	2	408698	5	NULL	NULL	0	NULL	literature 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of the literature on burns and trauma , October 1960 to August 1961 .
	manualset3
141265	3	408698	5	NULL	NULL	0	NULL	burns 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of the literature on burns and trauma , October 1960 to August 1961 .
	manualset3
141266	4	408698	5	NULL	NULL	0	NULL	trauma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of the literature on burns and trauma , October 1960 to August 1961 .
	manualset3
141267	5	408698	5	NULL	NULL	0	NULL	October 1960	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of the literature on burns and trauma , October 1960 to August 1961 .
	manualset3
141268	6	408698	5	NULL	NULL	0	NULL	August 1961	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of the literature on burns and trauma , October 1960 to August 1961 .
	manualset3
141269	1	408699	5	NULL	NULL	0	NULL	all-cause standardized mortality ratio ( SMR )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The all-cause standardized mortality ratio ( SMR ) was 71 , but a statistically significant increased mortality was seen for cancers of the other lymphatic tissues ( SMR = 162 ) , a rubric which includes multiple myeloma and non-Hodgkin 's lymphomas .
	manualset3
141270	2	408699	5	NULL	NULL	0	NULL	71	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The all-cause standardized mortality ratio ( SMR ) was 71 , but a statistically significant increased mortality was seen for cancers of the other lymphatic tissues ( SMR = 162 ) , a rubric which includes multiple myeloma and non-Hodgkin 's lymphomas .
	manualset3
141271	3	408699	5	NULL	NULL	0	NULL	mortality 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The all-cause standardized mortality ratio ( SMR ) was 71 , but a statistically significant increased mortality was seen for cancers of the other lymphatic tissues ( SMR = 162 ) , a rubric which includes multiple myeloma and non-Hodgkin 's lymphomas .
	manualset3
141272	4	408699	5	NULL	NULL	0	NULL	cancers 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The all-cause standardized mortality ratio ( SMR ) was 71 , but a statistically significant increased mortality was seen for cancers of the other lymphatic tissues ( SMR = 162 ) , a rubric which includes multiple myeloma and non-Hodgkin 's lymphomas .
	manualset3
141273	5	408699	5	NULL	NULL	0	NULL	lymphatic tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The all-cause standardized mortality ratio ( SMR ) was 71 , but a statistically significant increased mortality was seen for cancers of the other lymphatic tissues ( SMR = 162 ) , a rubric which includes multiple myeloma and non-Hodgkin 's lymphomas .
	manualset3
141274	6	408699	5	NULL	NULL	0	NULL	SMR = 162	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The all-cause standardized mortality ratio ( SMR ) was 71 , but a statistically significant increased mortality was seen for cancers of the other lymphatic tissues ( SMR = 162 ) , a rubric which includes multiple myeloma and non-Hodgkin 's lymphomas .
	manualset3
141275	7	408699	5	NULL	NULL	0	NULL	rubric 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The all-cause standardized mortality ratio ( SMR ) was 71 , but a statistically significant increased mortality was seen for cancers of the other lymphatic tissues ( SMR = 162 ) , a rubric which includes multiple myeloma and non-Hodgkin 's lymphomas .
	manualset3
141276	8	408699	5	NULL	NULL	0	NULL	multiple myeloma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The all-cause standardized mortality ratio ( SMR ) was 71 , but a statistically significant increased mortality was seen for cancers of the other lymphatic tissues ( SMR = 162 ) , a rubric which includes multiple myeloma and non-Hodgkin 's lymphomas .
	manualset3
141277	9	408699	5	NULL	NULL	0	NULL	non-Hodgkin 's lymphomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The all-cause standardized mortality ratio ( SMR ) was 71 , but a statistically significant increased mortality was seen for cancers of the other lymphatic tissues ( SMR = 162 ) , a rubric which includes multiple myeloma and non-Hodgkin 's lymphomas .
	manualset3
141278	1	408700	5	NULL	NULL	0	NULL	allelic frequencies	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The allelic frequencies of the 15 STR loci ( D8S1179 , D21S11 , D7S820 , CSF1PO , D3S1358 , TH01 , D13S317 , D16S539 , D2S1338 , D19S433 , vWA , TPOX , D18S51 , D5S818 and FGA ) were obtained from 2975 unrelated healthy Hui individuals .
	manualset3
141279	2	408700	5	NULL	NULL	0	NULL	15 STR loci 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The allelic frequencies of the 15 STR loci ( D8S1179 , D21S11 , D7S820 , CSF1PO , D3S1358 , TH01 , D13S317 , D16S539 , D2S1338 , D19S433 , vWA , TPOX , D18S51 , D5S818 and FGA ) were obtained from 2975 unrelated healthy Hui individuals .
	manualset3
141280	3	408700	5	NULL	NULL	0	NULL	D8S1179 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The allelic frequencies of the 15 STR loci ( D8S1179 , D21S11 , D7S820 , CSF1PO , D3S1358 , TH01 , D13S317 , D16S539 , D2S1338 , D19S433 , vWA , TPOX , D18S51 , D5S818 and FGA ) were obtained from 2975 unrelated healthy Hui individuals .
	manualset3
141281	4	408700	5	NULL	NULL	0	NULL	D21S11 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The allelic frequencies of the 15 STR loci ( D8S1179 , D21S11 , D7S820 , CSF1PO , D3S1358 , TH01 , D13S317 , D16S539 , D2S1338 , D19S433 , vWA , TPOX , D18S51 , D5S818 and FGA ) were obtained from 2975 unrelated healthy Hui individuals .
	manualset3
141282	5	408700	5	NULL	NULL	0	NULL	D7S820 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The allelic frequencies of the 15 STR loci ( D8S1179 , D21S11 , D7S820 , CSF1PO , D3S1358 , TH01 , D13S317 , D16S539 , D2S1338 , D19S433 , vWA , TPOX , D18S51 , D5S818 and FGA ) were obtained from 2975 unrelated healthy Hui individuals .
	manualset3
141283	6	408700	5	NULL	NULL	0	NULL	CSF1PO 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The allelic frequencies of the 15 STR loci ( D8S1179 , D21S11 , D7S820 , CSF1PO , D3S1358 , TH01 , D13S317 , D16S539 , D2S1338 , D19S433 , vWA , TPOX , D18S51 , D5S818 and FGA ) were obtained from 2975 unrelated healthy Hui individuals .
	manualset3
141284	7	408700	5	NULL	NULL	0	NULL	D3S1358 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The allelic frequencies of the 15 STR loci ( D8S1179 , D21S11 , D7S820 , CSF1PO , D3S1358 , TH01 , D13S317 , D16S539 , D2S1338 , D19S433 , vWA , TPOX , D18S51 , D5S818 and FGA ) were obtained from 2975 unrelated healthy Hui individuals .
	manualset3
141285	8	408700	5	NULL	NULL	0	NULL	TH01 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The allelic frequencies of the 15 STR loci ( D8S1179 , D21S11 , D7S820 , CSF1PO , D3S1358 , TH01 , D13S317 , D16S539 , D2S1338 , D19S433 , vWA , TPOX , D18S51 , D5S818 and FGA ) were obtained from 2975 unrelated healthy Hui individuals .
	manualset3
141286	9	408700	5	NULL	NULL	0	NULL	D13S317 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The allelic frequencies of the 15 STR loci ( D8S1179 , D21S11 , D7S820 , CSF1PO , D3S1358 , TH01 , D13S317 , D16S539 , D2S1338 , D19S433 , vWA , TPOX , D18S51 , D5S818 and FGA ) were obtained from 2975 unrelated healthy Hui individuals .
	manualset3
141287	10	408700	5	NULL	NULL	0	NULL	D16S539 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The allelic frequencies of the 15 STR loci ( D8S1179 , D21S11 , D7S820 , CSF1PO , D3S1358 , TH01 , D13S317 , D16S539 , D2S1338 , D19S433 , vWA , TPOX , D18S51 , D5S818 and FGA ) were obtained from 2975 unrelated healthy Hui individuals .
	manualset3
141288	11	408700	5	NULL	NULL	0	NULL	D2S1338 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The allelic frequencies of the 15 STR loci ( D8S1179 , D21S11 , D7S820 , CSF1PO , D3S1358 , TH01 , D13S317 , D16S539 , D2S1338 , D19S433 , vWA , TPOX , D18S51 , D5S818 and FGA ) were obtained from 2975 unrelated healthy Hui individuals .
	manualset3
141289	12	408700	5	NULL	NULL	0	NULL	D19S433 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The allelic frequencies of the 15 STR loci ( D8S1179 , D21S11 , D7S820 , CSF1PO , D3S1358 , TH01 , D13S317 , D16S539 , D2S1338 , D19S433 , vWA , TPOX , D18S51 , D5S818 and FGA ) were obtained from 2975 unrelated healthy Hui individuals .
	manualset3
141290	13	408700	5	NULL	NULL	0	NULL	vWA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The allelic frequencies of the 15 STR loci ( D8S1179 , D21S11 , D7S820 , CSF1PO , D3S1358 , TH01 , D13S317 , D16S539 , D2S1338 , D19S433 , vWA , TPOX , D18S51 , D5S818 and FGA ) were obtained from 2975 unrelated healthy Hui individuals .
	manualset3
141291	14	408700	5	NULL	NULL	0	NULL	TPOX 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The allelic frequencies of the 15 STR loci ( D8S1179 , D21S11 , D7S820 , CSF1PO , D3S1358 , TH01 , D13S317 , D16S539 , D2S1338 , D19S433 , vWA , TPOX , D18S51 , D5S818 and FGA ) were obtained from 2975 unrelated healthy Hui individuals .
	manualset3
141292	15	408700	5	NULL	NULL	0	NULL	D18S51 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The allelic frequencies of the 15 STR loci ( D8S1179 , D21S11 , D7S820 , CSF1PO , D3S1358 , TH01 , D13S317 , D16S539 , D2S1338 , D19S433 , vWA , TPOX , D18S51 , D5S818 and FGA ) were obtained from 2975 unrelated healthy Hui individuals .
	manualset3
141293	16	408700	5	NULL	NULL	0	NULL	D5S818 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The allelic frequencies of the 15 STR loci ( D8S1179 , D21S11 , D7S820 , CSF1PO , D3S1358 , TH01 , D13S317 , D16S539 , D2S1338 , D19S433 , vWA , TPOX , D18S51 , D5S818 and FGA ) were obtained from 2975 unrelated healthy Hui individuals .
	manualset3
141294	17	408700	5	NULL	NULL	0	NULL	FGA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The allelic frequencies of the 15 STR loci ( D8S1179 , D21S11 , D7S820 , CSF1PO , D3S1358 , TH01 , D13S317 , D16S539 , D2S1338 , D19S433 , vWA , TPOX , D18S51 , D5S818 and FGA ) were obtained from 2975 unrelated healthy Hui individuals .
	manualset3
141295	18	408700	5	NULL	NULL	0	NULL	2975 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The allelic frequencies of the 15 STR loci ( D8S1179 , D21S11 , D7S820 , CSF1PO , D3S1358 , TH01 , D13S317 , D16S539 , D2S1338 , D19S433 , vWA , TPOX , D18S51 , D5S818 and FGA ) were obtained from 2975 unrelated healthy Hui individuals .
	manualset3
141296	19	408700	5	NULL	NULL	0	NULL	healthy Hui individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The allelic frequencies of the 15 STR loci ( D8S1179 , D21S11 , D7S820 , CSF1PO , D3S1358 , TH01 , D13S317 , D16S539 , D2S1338 , D19S433 , vWA , TPOX , D18S51 , D5S818 and FGA ) were obtained from 2975 unrelated healthy Hui individuals .
	manualset3
141297	1	408701	5	NULL	NULL	0	NULL	surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The allocated surgery will then be performed with the preferred technique of the surgeon .
	manualset3
141298	2	408701	5	NULL	NULL	0	NULL	preferred technique	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The allocated surgery will then be performed with the preferred technique of the surgeon .
	manualset3
141299	3	408701	5	NULL	NULL	0	NULL	surgeon 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The allocated surgery will then be performed with the preferred technique of the surgeon .
	manualset3
141300	1	408702	5	NULL	NULL	0	NULL	alpha chain	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The alpha chain has the highest mobility , the beta chain has a slower mobility than the gamma chain , while the delta chain has about the same mobility as the beta chain .
	manualset3
141301	2	408702	5	NULL	NULL	0	NULL	mobility 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The alpha chain has the highest mobility , the beta chain has a slower mobility than the gamma chain , while the delta chain has about the same mobility as the beta chain .
	manualset3
141302	3	408702	5	NULL	NULL	0	NULL	 beta chain	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The alpha chain has the highest mobility , the beta chain has a slower mobility than the gamma chain , while the delta chain has about the same mobility as the beta chain .
	manualset3
141303	4	408702	5	NULL	NULL	0	NULL	mobility 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The alpha chain has the highest mobility , the beta chain has a slower mobility than the gamma chain , while the delta chain has about the same mobility as the beta chain .
	manualset3
141304	5	408702	5	NULL	NULL	0	NULL	gamma chain 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The alpha chain has the highest mobility , the beta chain has a slower mobility than the gamma chain , while the delta chain has about the same mobility as the beta chain .
	manualset3
141305	6	408702	5	NULL	NULL	0	NULL	delta chain 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The alpha chain has the highest mobility , the beta chain has a slower mobility than the gamma chain , while the delta chain has about the same mobility as the beta chain .
	manualset3
141306	7	408702	5	NULL	NULL	0	NULL	mobility 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The alpha chain has the highest mobility , the beta chain has a slower mobility than the gamma chain , while the delta chain has about the same mobility as the beta chain .
	manualset3
141307	8	408702	5	NULL	NULL	0	NULL	beta chain 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The alpha chain has the highest mobility , the beta chain has a slower mobility than the gamma chain , while the delta chain has about the same mobility as the beta chain .
	manualset3
141308	1	408703	5	NULL	NULL	0	NULL	 alpha65 mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The alpha65 mutation is shown to broaden the spectrum of amino acids permissible at P8 of the peptide .
	manualset3
141309	2	408703	5	NULL	NULL	0	NULL	spectrum 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The alpha65 mutation is shown to broaden the spectrum of amino acids permissible at P8 of the peptide .
	manualset3
141310	3	408703	5	NULL	NULL	0	NULL	amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The alpha65 mutation is shown to broaden the spectrum of amino acids permissible at P8 of the peptide .
	manualset3
141311	4	408703	5	NULL	NULL	0	NULL	 P8	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The alpha65 mutation is shown to broaden the spectrum of amino acids permissible at P8 of the peptide .
	manualset3
141312	5	408703	5	NULL	NULL	0	NULL	peptide 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The alpha65 mutation is shown to broaden the spectrum of amino acids permissible at P8 of the peptide .
	manualset3
141313	1	408704	5	NULL	NULL	0	NULL	alteration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The alteration during and the recovery of HEM after iontophoresis was also investigated .
	manualset3
141314	2	408704	5	NULL	NULL	0	NULL	recovery 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The alteration during and the recovery of HEM after iontophoresis was also investigated .
	manualset3
141315	3	408704	5	NULL	NULL	0	NULL	HEM 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The alteration during and the recovery of HEM after iontophoresis was also investigated .
	manualset3
141316	4	408704	5	NULL	NULL	0	NULL	iontophoresis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The alteration during and the recovery of HEM after iontophoresis was also investigated .
	manualset3
141317	1	408705	5	NULL	NULL	0	NULL	 iron concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The altered iron concentration in many neurodegenerative diseases such as Alzheimer 's disease ( AD ) has led to the development of MRI sequences that are sensitive to the accompanying changes in the transverse relaxation rate .
	manualset3
141318	2	408705	5	NULL	NULL	0	NULL	neurodegenerative diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The altered iron concentration in many neurodegenerative diseases such as Alzheimer 's disease ( AD ) has led to the development of MRI sequences that are sensitive to the accompanying changes in the transverse relaxation rate .
	manualset3
141319	3	408705	5	NULL	NULL	0	NULL	Alzheimer 's disease ( AD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The altered iron concentration in many neurodegenerative diseases such as Alzheimer 's disease ( AD ) has led to the development of MRI sequences that are sensitive to the accompanying changes in the transverse relaxation rate .
	manualset3
141320	4	408705	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The altered iron concentration in many neurodegenerative diseases such as Alzheimer 's disease ( AD ) has led to the development of MRI sequences that are sensitive to the accompanying changes in the transverse relaxation rate .
	manualset3
141321	5	408705	5	NULL	NULL	0	NULL	MRI sequences	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The altered iron concentration in many neurodegenerative diseases such as Alzheimer 's disease ( AD ) has led to the development of MRI sequences that are sensitive to the accompanying changes in the transverse relaxation rate .
	manualset3
141322	6	408705	5	NULL	NULL	0	NULL	accompanying changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The altered iron concentration in many neurodegenerative diseases such as Alzheimer 's disease ( AD ) has led to the development of MRI sequences that are sensitive to the accompanying changes in the transverse relaxation rate .
	manualset3
141323	7	408705	5	NULL	NULL	0	NULL	transverse relaxation rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The altered iron concentration in many neurodegenerative diseases such as Alzheimer 's disease ( AD ) has led to the development of MRI sequences that are sensitive to the accompanying changes in the transverse relaxation rate .
	manualset3
141324	1	408706	5	NULL	NULL	0	NULL	alveolar macrophages 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The alveolar macrophages were not activated as indicated by no change in expression of CD14 , CD16 , CD54 , CD95 , and scavenger receptor class A types I and II after surfactant treatment .
	manualset3
141325	2	408706	5	NULL	NULL	0	NULL	change 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The alveolar macrophages were not activated as indicated by no change in expression of CD14 , CD16 , CD54 , CD95 , and scavenger receptor class A types I and II after surfactant treatment .
	manualset3
141326	3	408706	5	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The alveolar macrophages were not activated as indicated by no change in expression of CD14 , CD16 , CD54 , CD95 , and scavenger receptor class A types I and II after surfactant treatment .
	manualset3
141327	4	408706	5	NULL	NULL	0	NULL	CD14 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The alveolar macrophages were not activated as indicated by no change in expression of CD14 , CD16 , CD54 , CD95 , and scavenger receptor class A types I and II after surfactant treatment .
	manualset3
141328	5	408706	5	NULL	NULL	0	NULL	CD16 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The alveolar macrophages were not activated as indicated by no change in expression of CD14 , CD16 , CD54 , CD95 , and scavenger receptor class A types I and II after surfactant treatment .
	manualset3
141329	6	408706	5	NULL	NULL	0	NULL	CD54 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The alveolar macrophages were not activated as indicated by no change in expression of CD14 , CD16 , CD54 , CD95 , and scavenger receptor class A types I and II after surfactant treatment .
	manualset3
141330	7	408706	5	NULL	NULL	0	NULL	CD95 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The alveolar macrophages were not activated as indicated by no change in expression of CD14 , CD16 , CD54 , CD95 , and scavenger receptor class A types I and II after surfactant treatment .
	manualset3
141331	8	408706	5	NULL	NULL	0	NULL	scavenger receptor class A type I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The alveolar macrophages were not activated as indicated by no change in expression of CD14 , CD16 , CD54 , CD95 , and scavenger receptor class A types I and II after surfactant treatment .
	manualset3
141332	9	408706	5	NULL	NULL	0	NULL	scavenger receptor class A type II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The alveolar macrophages were not activated as indicated by no change in expression of CD14 , CD16 , CD54 , CD95 , and scavenger receptor class A types I and II after surfactant treatment .
	manualset3
141333	10	408706	5	NULL	NULL	0	NULL	surfactant treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The alveolar macrophages were not activated as indicated by no change in expression of CD14 , CD16 , CD54 , CD95 , and scavenger receptor class A types I and II after surfactant treatment .
	manualset3
141334	1	408707	5	NULL	NULL	0	NULL	ambient pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ambient pH of these niches varies considerably , and therefore we have examined the response of C. glabrata to changes in ambient pH using a proteomic approach .
	manualset3
141335	2	408707	5	NULL	NULL	0	NULL	niches 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The ambient pH of these niches varies considerably , and therefore we have examined the response of C. glabrata to changes in ambient pH using a proteomic approach .
	manualset3
141336	3	408707	5	NULL	NULL	0	NULL	response 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ambient pH of these niches varies considerably , and therefore we have examined the response of C. glabrata to changes in ambient pH using a proteomic approach .
	manualset3
141337	4	408707	5	NULL	NULL	0	NULL	C. glabrata 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The ambient pH of these niches varies considerably , and therefore we have examined the response of C. glabrata to changes in ambient pH using a proteomic approach .
	manualset3
141338	5	408707	5	NULL	NULL	0	NULL	changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ambient pH of these niches varies considerably , and therefore we have examined the response of C. glabrata to changes in ambient pH using a proteomic approach .
	manualset3
141339	6	408707	5	NULL	NULL	0	NULL	ambient pH 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ambient pH of these niches varies considerably , and therefore we have examined the response of C. glabrata to changes in ambient pH using a proteomic approach .
	manualset3
141340	7	408707	5	NULL	NULL	0	NULL	proteomic approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ambient pH of these niches varies considerably , and therefore we have examined the response of C. glabrata to changes in ambient pH using a proteomic approach .
	manualset3
141341	1	408708	5	NULL	NULL	0	NULL	ameloblasts 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The ameloblasts expressed laminin gamma2 intensely throughout the period of active enamel deposition .
	manualset3
141342	2	408708	5	NULL	NULL	0	NULL	laminin gamma2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The ameloblasts expressed laminin gamma2 intensely throughout the period of active enamel deposition .
	manualset3
141343	3	408708	5	NULL	NULL	0	NULL	period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The ameloblasts expressed laminin gamma2 intensely throughout the period of active enamel deposition .
	manualset3
141344	4	408708	5	NULL	NULL	0	NULL	active enamel deposition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ameloblasts expressed laminin gamma2 intensely throughout the period of active enamel deposition .
	manualset3
141345	1	408709	5	NULL	NULL	0	NULL	amino-terminal sequence	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino-terminal sequence of all ten kappa-chains was characteristic for kappa III proteins and virtually identical to that of a prototype kappa III light chain .
	manualset3
141346	2	408709	5	NULL	NULL	0	NULL	ten 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino-terminal sequence of all ten kappa-chains was characteristic for kappa III proteins and virtually identical to that of a prototype kappa III light chain .
	manualset3
141347	3	408709	5	NULL	NULL	0	NULL	kappa-chains	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino-terminal sequence of all ten kappa-chains was characteristic for kappa III proteins and virtually identical to that of a prototype kappa III light chain .
	manualset3
141348	4	408709	5	NULL	NULL	0	NULL	kappa III proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino-terminal sequence of all ten kappa-chains was characteristic for kappa III proteins and virtually identical to that of a prototype kappa III light chain .
	manualset3
141349	5	408709	5	NULL	NULL	0	NULL	prototype kappa III light chain	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino-terminal sequence of all ten kappa-chains was characteristic for kappa III proteins and virtually identical to that of a prototype kappa III light chain .
	manualset3
141350	1	408710	5	NULL	NULL	0	NULL	amino acid composition	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino acid composition of AMP5 and sequence of the N-terminal 50 amino acid residues was determined .
	manualset3
141351	2	408710	5	NULL	NULL	0	NULL	AMP5 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino acid composition of AMP5 and sequence of the N-terminal 50 amino acid residues was determined .
	manualset3
141352	3	408710	5	NULL	NULL	0	NULL	sequence 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino acid composition of AMP5 and sequence of the N-terminal 50 amino acid residues was determined .
	manualset3
141353	4	408710	5	NULL	NULL	0	NULL	N-terminal 50 amino acid residues	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino acid composition of AMP5 and sequence of the N-terminal 50 amino acid residues was determined .
	manualset3
141354	1	408711	5	NULL	NULL	NULL	NULL	amino acid sequence	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The amino acid sequence of a high-redox-potential ferredoxin from the purple phototrophic bacterium , Rhodospirillum tenue strain 2761 .
	manualset3
141355	2	408711	5	NULL	NULL	0	NULL	high-redox-potential ferredoxin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino acid sequence of a high-redox-potential ferredoxin from the purple phototrophic bacterium , Rhodospirillum tenue strain 2761 .
	manualset3
141356	3	408711	5	NULL	NULL	0	NULL	purple phototrophic bacterium , Rhodospirillum tenue strain 2761	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino acid sequence of a high-redox-potential ferredoxin from the purple phototrophic bacterium , Rhodospirillum tenue strain 2761 .
	manualset3
141357	1	408712	5	NULL	NULL	0	NULL	amino acid sequence 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino acid sequence of the Cry2Ab25 protein was compared with previously known Cry2Ab toxins , and the phylogenetic relationships among them were determined .
	manualset3
141358	2	408712	5	NULL	NULL	0	NULL	Cry2Ab25 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino acid sequence of the Cry2Ab25 protein was compared with previously known Cry2Ab toxins , and the phylogenetic relationships among them were determined .
	manualset3
141359	3	408712	5	NULL	NULL	0	NULL	Cry2Ab toxins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino acid sequence of the Cry2Ab25 protein was compared with previously known Cry2Ab toxins , and the phylogenetic relationships among them were determined .
	manualset3
141360	4	408712	5	NULL	NULL	0	NULL	phylogenetic relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino acid sequence of the Cry2Ab25 protein was compared with previously known Cry2Ab toxins , and the phylogenetic relationships among them were determined .
	manualset3
141361	1	408713	5	NULL	NULL	0	NULL	amino acid sequence	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino acid sequence of the membrane glycoprotein of Sindbis virus is specified by the viral genome , but it has not been determined whether the carbohydrate portion of this molecule is specified by the cell or by the virus .
	manualset3
141362	2	408713	5	NULL	NULL	0	NULL	membrane glycoprotein	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino acid sequence of the membrane glycoprotein of Sindbis virus is specified by the viral genome , but it has not been determined whether the carbohydrate portion of this molecule is specified by the cell or by the virus .
	manualset3
141363	3	408713	5	NULL	NULL	0	NULL	Sindbis virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino acid sequence of the membrane glycoprotein of Sindbis virus is specified by the viral genome , but it has not been determined whether the carbohydrate portion of this molecule is specified by the cell or by the virus .
	manualset3
141364	4	408713	5	NULL	NULL	0	NULL	viral genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino acid sequence of the membrane glycoprotein of Sindbis virus is specified by the viral genome , but it has not been determined whether the carbohydrate portion of this molecule is specified by the cell or by the virus .
	manualset3
141365	5	408713	5	NULL	NULL	0	NULL	carbohydrate portion	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino acid sequence of the membrane glycoprotein of Sindbis virus is specified by the viral genome , but it has not been determined whether the carbohydrate portion of this molecule is specified by the cell or by the virus .
	manualset3
141366	6	408713	5	NULL	NULL	0	NULL	molecule 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino acid sequence of the membrane glycoprotein of Sindbis virus is specified by the viral genome , but it has not been determined whether the carbohydrate portion of this molecule is specified by the cell or by the virus .
	manualset3
141367	7	408713	5	NULL	NULL	0	NULL	cell 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino acid sequence of the membrane glycoprotein of Sindbis virus is specified by the viral genome , but it has not been determined whether the carbohydrate portion of this molecule is specified by the cell or by the virus .
	manualset3
141368	8	408713	5	NULL	NULL	0	NULL	virus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino acid sequence of the membrane glycoprotein of Sindbis virus is specified by the viral genome , but it has not been determined whether the carbohydrate portion of this molecule is specified by the cell or by the virus .
	manualset3
141369	1	408714	5	NULL	NULL	0	NULL	 amino acid sequence requirements 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino acid sequence requirements for the hydrolysis of ceftazidime , an extended spectrum cephalosporin commonly used to treat serious infections , were determined by selecting resistant mutants from each of the 21 libraries .
	manualset3
141370	2	408714	5	NULL	NULL	0	NULL	hydrolysis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino acid sequence requirements for the hydrolysis of ceftazidime , an extended spectrum cephalosporin commonly used to treat serious infections , were determined by selecting resistant mutants from each of the 21 libraries .
	manualset3
141371	3	408714	5	NULL	NULL	NULL	NULL	ceftazidime , an extended spectrum cephalosporin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The amino acid sequence requirements for the hydrolysis of ceftazidime , an extended spectrum cephalosporin commonly used to treat serious infections , were determined by selecting resistant mutants from each of the 21 libraries .
	manualset3
141372	4	408714	5	NULL	NULL	0	NULL	serious infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino acid sequence requirements for the hydrolysis of ceftazidime , an extended spectrum cephalosporin commonly used to treat serious infections , were determined by selecting resistant mutants from each of the 21 libraries .
	manualset3
141373	5	408714	5	NULL	NULL	NULL	NULL	resistant mutants	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The amino acid sequence requirements for the hydrolysis of ceftazidime , an extended spectrum cephalosporin commonly used to treat serious infections , were determined by selecting resistant mutants from each of the 21 libraries .
	manualset3
141374	6	408714	5	NULL	NULL	0	NULL	21 libraries	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino acid sequence requirements for the hydrolysis of ceftazidime , an extended spectrum cephalosporin commonly used to treat serious infections , were determined by selecting resistant mutants from each of the 21 libraries .
	manualset3
141375	1	408715	5	NULL	NULL	0	NULL	amino acid sequences	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino acid sequences of subunits alpha and beta in the pig were , respectively , 98 and 96 % identical to those in humans .
	manualset3
141376	2	408715	5	NULL	NULL	0	NULL	subunit alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino acid sequences of subunits alpha and beta in the pig were , respectively , 98 and 96 % identical to those in humans .
	manualset3
141377	3	408715	5	NULL	NULL	0	NULL	subunit beta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino acid sequences of subunits alpha and beta in the pig were , respectively , 98 and 96 % identical to those in humans .
	manualset3
141378	4	408715	5	NULL	NULL	0	NULL	pig 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino acid sequences of subunits alpha and beta in the pig were , respectively , 98 and 96 % identical to those in humans .
	manualset3
141379	5	408715	5	NULL	NULL	0	NULL	98 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino acid sequences of subunits alpha and beta in the pig were , respectively , 98 and 96 % identical to those in humans .
	manualset3
141380	6	408715	5	NULL	NULL	0	NULL	96 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino acid sequences of subunits alpha and beta in the pig were , respectively , 98 and 96 % identical to those in humans .
	manualset3
141381	7	408715	5	NULL	NULL	0	NULL	humans 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino acid sequences of subunits alpha and beta in the pig were , respectively , 98 and 96 % identical to those in humans .
	manualset3
141382	1	408716	5	NULL	NULL	0	NULL	ammonia load	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ammonia load started at a nitrogen-loading rate of 0.02 kg m ( -3 ) day ( -1 ) and was increased stepwise .
	manualset3
141383	2	408716	5	NULL	NULL	0	NULL	nitrogen-loading rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ammonia load started at a nitrogen-loading rate of 0.02 kg m ( -3 ) day ( -1 ) and was increased stepwise .
	manualset3
141384	3	408716	5	NULL	NULL	0	NULL	0.02 kg m ( -3 ) day ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ammonia load started at a nitrogen-loading rate of 0.02 kg m ( -3 ) day ( -1 ) and was increased stepwise .
	manualset3
141385	1	408717	5	NULL	NULL	0	NULL	amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of ODC-mRNA formed after growth stimulation was not affected by 6P .
	manualset3
141386	2	408717	5	NULL	NULL	0	NULL	ODC-mRNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of ODC-mRNA formed after growth stimulation was not affected by 6P .
	manualset3
141387	3	408717	5	NULL	NULL	0	NULL	growth stimulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of ODC-mRNA formed after growth stimulation was not affected by 6P .
	manualset3
141388	4	408717	5	NULL	NULL	0	NULL	6P	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of ODC-mRNA formed after growth stimulation was not affected by 6P .
	manualset3
141389	1	408718	5	NULL	NULL	0	NULL	amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of TR mRNA , which was not affected in PTU treated mice , was increased only after T3 treatment as observed in overt hypothyroidism .
	manualset3
141390	2	408718	5	NULL	NULL	0	NULL	TR mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of TR mRNA , which was not affected in PTU treated mice , was increased only after T3 treatment as observed in overt hypothyroidism .
	manualset3
141391	3	408718	5	NULL	NULL	0	NULL	PTU treated mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of TR mRNA , which was not affected in PTU treated mice , was increased only after T3 treatment as observed in overt hypothyroidism .
	manualset3
141392	4	408718	5	NULL	NULL	0	NULL	T3 treatment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of TR mRNA , which was not affected in PTU treated mice , was increased only after T3 treatment as observed in overt hypothyroidism .
	manualset3
141393	5	408718	5	NULL	NULL	0	NULL	hypothyroidism 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of TR mRNA , which was not affected in PTU treated mice , was increased only after T3 treatment as observed in overt hypothyroidism .
	manualset3
141394	1	408719	5	NULL	NULL	0	NULL	amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of bone forming osteoblasts was also significantly greater in the psoralen group than the negative control -- collagen group .
	manualset3
141395	2	408719	5	NULL	NULL	0	NULL	bone forming osteoblasts 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of bone forming osteoblasts was also significantly greater in the psoralen group than the negative control -- collagen group .
	manualset3
141396	3	408719	5	NULL	NULL	0	NULL	psoralen group 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of bone forming osteoblasts was also significantly greater in the psoralen group than the negative control -- collagen group .
	manualset3
141397	4	408719	5	NULL	NULL	0	NULL	negative control -- collagen group	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of bone forming osteoblasts was also significantly greater in the psoralen group than the negative control -- collagen group .
	manualset3
141398	1	408720	5	NULL	NULL	0	NULL	amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of fluid removed was closely related to changes in Ppl , sw and PEEPi .
	manualset3
141399	2	408720	5	NULL	NULL	0	NULL	fluid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of fluid removed was closely related to changes in Ppl , sw and PEEPi .
	manualset3
141400	3	408720	5	NULL	NULL	0	NULL	changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of fluid removed was closely related to changes in Ppl , sw and PEEPi .
	manualset3
141401	4	408720	5	NULL	NULL	0	NULL	Ppl , sw	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of fluid removed was closely related to changes in Ppl , sw and PEEPi .
	manualset3
141402	5	408720	5	NULL	NULL	0	NULL	PEEPi 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of fluid removed was closely related to changes in Ppl , sw and PEEPi .
	manualset3
141403	1	408721	5	NULL	NULL	0	NULL	amount 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of glucose in the supplement was 0.5 g ( 1 % the amount of glucose used in adult studies of cognitive functioning and memory ) .
	manualset3
141404	2	408721	5	NULL	NULL	0	NULL	glucose 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of glucose in the supplement was 0.5 g ( 1 % the amount of glucose used in adult studies of cognitive functioning and memory ) .
	manualset3
141405	3	408721	5	NULL	NULL	0	NULL	supplement 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of glucose in the supplement was 0.5 g ( 1 % the amount of glucose used in adult studies of cognitive functioning and memory ) .
	manualset3
141406	4	408721	5	NULL	NULL	0	NULL	0.5 g	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of glucose in the supplement was 0.5 g ( 1 % the amount of glucose used in adult studies of cognitive functioning and memory ) .
	manualset3
141407	5	408721	5	NULL	NULL	0	NULL	1 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of glucose in the supplement was 0.5 g ( 1 % the amount of glucose used in adult studies of cognitive functioning and memory ) .
	manualset3
141408	6	408721	5	NULL	NULL	0	NULL	amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of glucose in the supplement was 0.5 g ( 1 % the amount of glucose used in adult studies of cognitive functioning and memory ) .
	manualset3
141409	7	408721	5	NULL	NULL	0	NULL	glucose 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of glucose in the supplement was 0.5 g ( 1 % the amount of glucose used in adult studies of cognitive functioning and memory ) .
	manualset3
141410	8	408721	5	NULL	NULL	0	NULL	adult studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of glucose in the supplement was 0.5 g ( 1 % the amount of glucose used in adult studies of cognitive functioning and memory ) .
	manualset3
141411	9	408721	5	NULL	NULL	0	NULL	cognitive functioning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of glucose in the supplement was 0.5 g ( 1 % the amount of glucose used in adult studies of cognitive functioning and memory ) .
	manualset3
141412	10	408721	5	NULL	NULL	0	NULL	memory 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of glucose in the supplement was 0.5 g ( 1 % the amount of glucose used in adult studies of cognitive functioning and memory ) .
	manualset3
141413	1	408722	5	NULL	NULL	0	NULL	amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of labeled steroid bound by endotoxin-treated mice was 13 , 606 + / - 2 , 027 dpm/mg cytosol protein compared with 17 , 247 + / - 2 , 084 dpm/mg cytosol protein in adrenalectomized controls .
	manualset3
141414	2	408722	5	NULL	NULL	0	NULL	labeled steroid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of labeled steroid bound by endotoxin-treated mice was 13 , 606 + / - 2 , 027 dpm/mg cytosol protein compared with 17 , 247 + / - 2 , 084 dpm/mg cytosol protein in adrenalectomized controls .
	manualset3
141415	3	408722	5	NULL	NULL	0	NULL	endotoxin-treated mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of labeled steroid bound by endotoxin-treated mice was 13 , 606 + / - 2 , 027 dpm/mg cytosol protein compared with 17 , 247 + / - 2 , 084 dpm/mg cytosol protein in adrenalectomized controls .
	manualset3
141416	4	408722	5	NULL	NULL	NULL	NULL	13 , 606 + / - 2 , 027 dpm/mg 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The amount of labeled steroid bound by endotoxin-treated mice was 13 , 606 + / - 2 , 027 dpm/mg cytosol protein compared with 17 , 247 + / - 2 , 084 dpm/mg cytosol protein in adrenalectomized controls .
	manualset3
141417	5	408722	5	NULL	NULL	NULL	NULL	cytosol protein 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The amount of labeled steroid bound by endotoxin-treated mice was 13 , 606 + / - 2 , 027 dpm/mg cytosol protein compared with 17 , 247 + / - 2 , 084 dpm/mg cytosol protein in adrenalectomized controls .
	manualset3
141418	6	408722	5	NULL	NULL	0	NULL	17 , 247 + / - 2 , 084 dpm/mg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of labeled steroid bound by endotoxin-treated mice was 13 , 606 + / - 2 , 027 dpm/mg cytosol protein compared with 17 , 247 + / - 2 , 084 dpm/mg cytosol protein in adrenalectomized controls .
	manualset3
141419	7	408722	5	NULL	NULL	0	NULL	cytosol protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of labeled steroid bound by endotoxin-treated mice was 13 , 606 + / - 2 , 027 dpm/mg cytosol protein compared with 17 , 247 + / - 2 , 084 dpm/mg cytosol protein in adrenalectomized controls .
	manualset3
141420	8	408722	5	NULL	NULL	0	NULL	adrenalectomized controls	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of labeled steroid bound by endotoxin-treated mice was 13 , 606 + / - 2 , 027 dpm/mg cytosol protein compared with 17 , 247 + / - 2 , 084 dpm/mg cytosol protein in adrenalectomized controls .
	manualset3
141421	1	408723	5	NULL	NULL	0	NULL	amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of test substance that produced 20 % leakage compared with a cell-free control was determined ( FL ( 20 ) H4 ) .
	manualset3
141422	2	408723	5	NULL	NULL	0	NULL	test substance 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of test substance that produced 20 % leakage compared with a cell-free control was determined ( FL ( 20 ) H4 ) .
	manualset3
141423	3	408723	5	NULL	NULL	0	NULL	 20 % leakage	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of test substance that produced 20 % leakage compared with a cell-free control was determined ( FL ( 20 ) H4 ) .
	manualset3
141424	4	408723	5	NULL	NULL	0	NULL	cell-free control	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of test substance that produced 20 % leakage compared with a cell-free control was determined ( FL ( 20 ) H4 ) .
	manualset3
141425	5	408723	5	NULL	NULL	0	NULL	 ( FL ( 20 ) H4 )	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of test substance that produced 20 % leakage compared with a cell-free control was determined ( FL ( 20 ) H4 ) .
	manualset3
141426	1	408724	5	NULL	NULL	0	NULL	amounts 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The amounts of the high-affinity binding sites for muscimol and GABA were similar ( Bmax = 1.7 and 1.5 pmol/mg protein , respectively ) .
	manualset3
141427	2	408724	5	NULL	NULL	0	NULL	high-affinity binding sites 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The amounts of the high-affinity binding sites for muscimol and GABA were similar ( Bmax = 1.7 and 1.5 pmol/mg protein , respectively ) .
	manualset3
141428	3	408724	5	NULL	NULL	NULL	NULL	muscimol 	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The amounts of the high-affinity binding sites for muscimol and GABA were similar ( Bmax = 1.7 and 1.5 pmol/mg protein , respectively ) .
	manualset3
141429	4	408724	5	NULL	NULL	0	NULL	GABA 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The amounts of the high-affinity binding sites for muscimol and GABA were similar ( Bmax = 1.7 and 1.5 pmol/mg protein , respectively ) .
	manualset3
141430	5	408724	5	NULL	NULL	0	NULL	Bmax = 1.7 and 1.5 pmol/mg protein	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The amounts of the high-affinity binding sites for muscimol and GABA were similar ( Bmax = 1.7 and 1.5 pmol/mg protein , respectively ) .
	manualset3
141431	1	408725	5	NULL	NULL	0	NULL	amplitude 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The amplitude of the CMS-CMAP ( 1.00 + / - 0.15 mV ) was much higher than that of ES-CMAP ( 0.26 + / - 0.15 mV ) when recorded from pair C. Good-quality CMS-CMAPs could be recorded in some subjects from an electrode positioned very low in the esophagus .
	manualset3
141432	2	408725	5	NULL	NULL	0	NULL	 CMS-CMAP	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The amplitude of the CMS-CMAP ( 1.00 + / - 0.15 mV ) was much higher than that of ES-CMAP ( 0.26 + / - 0.15 mV ) when recorded from pair C. Good-quality CMS-CMAPs could be recorded in some subjects from an electrode positioned very low in the esophagus .
	manualset3
141433	3	408725	5	NULL	NULL	0	NULL	1.00 + / - 0.15 mV	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The amplitude of the CMS-CMAP ( 1.00 + / - 0.15 mV ) was much higher than that of ES-CMAP ( 0.26 + / - 0.15 mV ) when recorded from pair C. Good-quality CMS-CMAPs could be recorded in some subjects from an electrode positioned very low in the esophagus .
	manualset3
141434	4	408725	5	NULL	NULL	0	NULL	ES-CMAP	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The amplitude of the CMS-CMAP ( 1.00 + / - 0.15 mV ) was much higher than that of ES-CMAP ( 0.26 + / - 0.15 mV ) when recorded from pair C. Good-quality CMS-CMAPs could be recorded in some subjects from an electrode positioned very low in the esophagus .
	manualset3
141435	5	408725	5	NULL	NULL	0	NULL	0.26 + / - 0.15 mV	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The amplitude of the CMS-CMAP ( 1.00 + / - 0.15 mV ) was much higher than that of ES-CMAP ( 0.26 + / - 0.15 mV ) when recorded from pair C. Good-quality CMS-CMAPs could be recorded in some subjects from an electrode positioned very low in the esophagus .
	manualset3
141436	6	408725	5	NULL	NULL	0	NULL	Good-quality CMS-CMAPs 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The amplitude of the CMS-CMAP ( 1.00 + / - 0.15 mV ) was much higher than that of ES-CMAP ( 0.26 + / - 0.15 mV ) when recorded from pair C. Good-quality CMS-CMAPs could be recorded in some subjects from an electrode positioned very low in the esophagus .
	manualset3
141437	7	408725	5	NULL	NULL	0	NULL	electrode	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The amplitude of the CMS-CMAP ( 1.00 + / - 0.15 mV ) was much higher than that of ES-CMAP ( 0.26 + / - 0.15 mV ) when recorded from pair C. Good-quality CMS-CMAPs could be recorded in some subjects from an electrode positioned very low in the esophagus .
	manualset3
141438	8	408725	5	NULL	NULL	0	NULL	esophagus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The amplitude of the CMS-CMAP ( 1.00 + / - 0.15 mV ) was much higher than that of ES-CMAP ( 0.26 + / - 0.15 mV ) when recorded from pair C. Good-quality CMS-CMAPs could be recorded in some subjects from an electrode positioned very low in the esophagus .
	manualset3
141439	1	408726	5	NULL	NULL	0	NULL	amplitudes 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The amplitudes of block caused by 50 microM AR-R15896AR , 10 microM ketamine , or 10 microM memantine were not significantly different , being 82 + / - 1 % , 80 + / - 2 % , and 81 + / - 2 % , respectively .
	manualset3
141440	2	408726	5	NULL	NULL	0	NULL	block 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The amplitudes of block caused by 50 microM AR-R15896AR , 10 microM ketamine , or 10 microM memantine were not significantly different , being 82 + / - 1 % , 80 + / - 2 % , and 81 + / - 2 % , respectively .
	manualset3
141441	3	408726	5	NULL	NULL	0	NULL	50 microM AR-R15896AR	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The amplitudes of block caused by 50 microM AR-R15896AR , 10 microM ketamine , or 10 microM memantine were not significantly different , being 82 + / - 1 % , 80 + / - 2 % , and 81 + / - 2 % , respectively .
	manualset3
141442	4	408726	5	NULL	NULL	0	NULL	10 microM ketamine	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The amplitudes of block caused by 50 microM AR-R15896AR , 10 microM ketamine , or 10 microM memantine were not significantly different , being 82 + / - 1 % , 80 + / - 2 % , and 81 + / - 2 % , respectively .
	manualset3
141443	5	408726	5	NULL	NULL	0	NULL	10 microM memantine	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The amplitudes of block caused by 50 microM AR-R15896AR , 10 microM ketamine , or 10 microM memantine were not significantly different , being 82 + / - 1 % , 80 + / - 2 % , and 81 + / - 2 % , respectively .
	manualset3
141444	6	408726	5	NULL	NULL	0	NULL	2 + / - 1 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The amplitudes of block caused by 50 microM AR-R15896AR , 10 microM ketamine , or 10 microM memantine were not significantly different , being 82 + / - 1 % , 80 + / - 2 % , and 81 + / - 2 % , respectively .
	manualset3
141445	7	408726	5	NULL	NULL	0	NULL	80 + / - 2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The amplitudes of block caused by 50 microM AR-R15896AR , 10 microM ketamine , or 10 microM memantine were not significantly different , being 82 + / - 1 % , 80 + / - 2 % , and 81 + / - 2 % , respectively .
	manualset3
141446	8	408726	5	NULL	NULL	0	NULL	81 + / - 2 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The amplitudes of block caused by 50 microM AR-R15896AR , 10 microM ketamine , or 10 microM memantine were not significantly different , being 82 + / - 1 % , 80 + / - 2 % , and 81 + / - 2 % , respectively .
	manualset3
141447	1	408727	5	NULL	NULL	0	NULL	review 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A review on the role of phytosterols : new insights into cardiovascular risk .
	manualset3
141448	2	408727	5	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A review on the role of phytosterols : new insights into cardiovascular risk .
	manualset3
141449	3	408727	5	NULL	NULL	0	NULL	phytosterols 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A review on the role of phytosterols : new insights into cardiovascular risk .
	manualset3
141450	4	408727	5	NULL	NULL	0	NULL	insights 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A review on the role of phytosterols : new insights into cardiovascular risk .
	manualset3
141451	5	408727	5	NULL	NULL	0	NULL	cardiovascular risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A review on the role of phytosterols : new insights into cardiovascular risk .
	manualset3
141452	1	408728	5	NULL	NULL	0	NULL	anaerobic organisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The anaerobic organisms tested were equally susceptible to both FCE 22101 and imipenem .
	manualset3
141453	2	408728	5	NULL	NULL	0	NULL	FCE 22101	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The anaerobic organisms tested were equally susceptible to both FCE 22101 and imipenem .
	manualset3
141454	3	408728	5	NULL	NULL	0	NULL	imipenem 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The anaerobic organisms tested were equally susceptible to both FCE 22101 and imipenem .
	manualset3
141455	1	408729	5	NULL	NULL	0	NULL	analgesic action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The analgesic action of THIP in the hot-plate test was not blocked by naloxone , bicuculline , phentolamine or methysergide , but was partially reversed by a high dose of atropine , indicating that classic opiate-receptors , bicuculline-sensitive GABA-receptors , alpha-adrenoceptors and serotonin-receptors do not appear to mediate the action of THIP but that cholinergic receptors might be indirectly involved .
	manualset3
141456	2	408729	5	NULL	NULL	0	NULL	THIP 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The analgesic action of THIP in the hot-plate test was not blocked by naloxone , bicuculline , phentolamine or methysergide , but was partially reversed by a high dose of atropine , indicating that classic opiate-receptors , bicuculline-sensitive GABA-receptors , alpha-adrenoceptors and serotonin-receptors do not appear to mediate the action of THIP but that cholinergic receptors might be indirectly involved .
	manualset3
141457	3	408729	5	NULL	NULL	0	NULL	hot-plate test 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The analgesic action of THIP in the hot-plate test was not blocked by naloxone , bicuculline , phentolamine or methysergide , but was partially reversed by a high dose of atropine , indicating that classic opiate-receptors , bicuculline-sensitive GABA-receptors , alpha-adrenoceptors and serotonin-receptors do not appear to mediate the action of THIP but that cholinergic receptors might be indirectly involved .
	manualset3
141458	4	408729	5	NULL	NULL	0	NULL	naloxone 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The analgesic action of THIP in the hot-plate test was not blocked by naloxone , bicuculline , phentolamine or methysergide , but was partially reversed by a high dose of atropine , indicating that classic opiate-receptors , bicuculline-sensitive GABA-receptors , alpha-adrenoceptors and serotonin-receptors do not appear to mediate the action of THIP but that cholinergic receptors might be indirectly involved .
	manualset3
141459	5	408729	5	NULL	NULL	0	NULL	bicuculline 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The analgesic action of THIP in the hot-plate test was not blocked by naloxone , bicuculline , phentolamine or methysergide , but was partially reversed by a high dose of atropine , indicating that classic opiate-receptors , bicuculline-sensitive GABA-receptors , alpha-adrenoceptors and serotonin-receptors do not appear to mediate the action of THIP but that cholinergic receptors might be indirectly involved .
	manualset3
141461	7	408729	5	NULL	NULL	0	NULL	phentolamine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The analgesic action of THIP in the hot-plate test was not blocked by naloxone , bicuculline , phentolamine or methysergide , but was partially reversed by a high dose of atropine , indicating that classic opiate-receptors , bicuculline-sensitive GABA-receptors , alpha-adrenoceptors and serotonin-receptors do not appear to mediate the action of THIP but that cholinergic receptors might be indirectly involved .
	manualset3
141462	8	408729	5	NULL	NULL	0	NULL	methysergide 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The analgesic action of THIP in the hot-plate test was not blocked by naloxone , bicuculline , phentolamine or methysergide , but was partially reversed by a high dose of atropine , indicating that classic opiate-receptors , bicuculline-sensitive GABA-receptors , alpha-adrenoceptors and serotonin-receptors do not appear to mediate the action of THIP but that cholinergic receptors might be indirectly involved .
	manualset3
141463	9	408729	5	NULL	NULL	0	NULL	dose 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The analgesic action of THIP in the hot-plate test was not blocked by naloxone , bicuculline , phentolamine or methysergide , but was partially reversed by a high dose of atropine , indicating that classic opiate-receptors , bicuculline-sensitive GABA-receptors , alpha-adrenoceptors and serotonin-receptors do not appear to mediate the action of THIP but that cholinergic receptors might be indirectly involved .
	manualset3
141464	10	408729	5	NULL	NULL	0	NULL	atropine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The analgesic action of THIP in the hot-plate test was not blocked by naloxone , bicuculline , phentolamine or methysergide , but was partially reversed by a high dose of atropine , indicating that classic opiate-receptors , bicuculline-sensitive GABA-receptors , alpha-adrenoceptors and serotonin-receptors do not appear to mediate the action of THIP but that cholinergic receptors might be indirectly involved .
	manualset3
141465	11	408729	5	NULL	NULL	0	NULL	classic opiate-receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The analgesic action of THIP in the hot-plate test was not blocked by naloxone , bicuculline , phentolamine or methysergide , but was partially reversed by a high dose of atropine , indicating that classic opiate-receptors , bicuculline-sensitive GABA-receptors , alpha-adrenoceptors and serotonin-receptors do not appear to mediate the action of THIP but that cholinergic receptors might be indirectly involved .
	manualset3
141466	12	408729	5	NULL	NULL	0	NULL	bicuculline-sensitive GABA-receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The analgesic action of THIP in the hot-plate test was not blocked by naloxone , bicuculline , phentolamine or methysergide , but was partially reversed by a high dose of atropine , indicating that classic opiate-receptors , bicuculline-sensitive GABA-receptors , alpha-adrenoceptors and serotonin-receptors do not appear to mediate the action of THIP but that cholinergic receptors might be indirectly involved .
	manualset3
141467	13	408729	5	NULL	NULL	0	NULL	alpha-adrenoceptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The analgesic action of THIP in the hot-plate test was not blocked by naloxone , bicuculline , phentolamine or methysergide , but was partially reversed by a high dose of atropine , indicating that classic opiate-receptors , bicuculline-sensitive GABA-receptors , alpha-adrenoceptors and serotonin-receptors do not appear to mediate the action of THIP but that cholinergic receptors might be indirectly involved .
	manualset3
141468	14	408729	5	NULL	NULL	0	NULL	serotonin-receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The analgesic action of THIP in the hot-plate test was not blocked by naloxone , bicuculline , phentolamine or methysergide , but was partially reversed by a high dose of atropine , indicating that classic opiate-receptors , bicuculline-sensitive GABA-receptors , alpha-adrenoceptors and serotonin-receptors do not appear to mediate the action of THIP but that cholinergic receptors might be indirectly involved .
	manualset3
141469	15	408729	5	NULL	NULL	0	NULL	action 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The analgesic action of THIP in the hot-plate test was not blocked by naloxone , bicuculline , phentolamine or methysergide , but was partially reversed by a high dose of atropine , indicating that classic opiate-receptors , bicuculline-sensitive GABA-receptors , alpha-adrenoceptors and serotonin-receptors do not appear to mediate the action of THIP but that cholinergic receptors might be indirectly involved .
	manualset3
141470	16	408729	5	NULL	NULL	0	NULL	THIP 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The analgesic action of THIP in the hot-plate test was not blocked by naloxone , bicuculline , phentolamine or methysergide , but was partially reversed by a high dose of atropine , indicating that classic opiate-receptors , bicuculline-sensitive GABA-receptors , alpha-adrenoceptors and serotonin-receptors do not appear to mediate the action of THIP but that cholinergic receptors might be indirectly involved .
	manualset3
141471	17	408729	5	NULL	NULL	0	NULL	cholinergic receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The analgesic action of THIP in the hot-plate test was not blocked by naloxone , bicuculline , phentolamine or methysergide , but was partially reversed by a high dose of atropine , indicating that classic opiate-receptors , bicuculline-sensitive GABA-receptors , alpha-adrenoceptors and serotonin-receptors do not appear to mediate the action of THIP but that cholinergic receptors might be indirectly involved .
	manualset3
141472	1	408730	5	NULL	NULL	0	NULL	analgesic effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The analgesic effect of tramadol after oral administration was decreased , which could be explained by the induction of tramadol metabolism in the liver , but should be examined in more details .
	manualset3
141473	2	408730	5	NULL	NULL	0	NULL	tramadol 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The analgesic effect of tramadol after oral administration was decreased , which could be explained by the induction of tramadol metabolism in the liver , but should be examined in more details .
	manualset3
141474	3	408730	5	NULL	NULL	0	NULL	oral administration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The analgesic effect of tramadol after oral administration was decreased , which could be explained by the induction of tramadol metabolism in the liver , but should be examined in more details .
	manualset3
141475	4	408730	5	NULL	NULL	0	NULL	induction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The analgesic effect of tramadol after oral administration was decreased , which could be explained by the induction of tramadol metabolism in the liver , but should be examined in more details .
	manualset3
141476	5	408730	5	NULL	NULL	0	NULL	tramadol metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The analgesic effect of tramadol after oral administration was decreased , which could be explained by the induction of tramadol metabolism in the liver , but should be examined in more details .
	manualset3
141477	6	408730	5	NULL	NULL	0	NULL	liver 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The analgesic effect of tramadol after oral administration was decreased , which could be explained by the induction of tramadol metabolism in the liver , but should be examined in more details .
	manualset3
141478	1	408731	5	NULL	NULL	0	NULL	users 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The analyses compared ( i ) users of anxiolytics with non-users and ( ii ) three groups of anxiolytic users classified according to pattern ( frequency and regularity ) of use .
	manualset3
141479	2	408731	5	NULL	NULL	0	NULL	anxiolytics 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The analyses compared ( i ) users of anxiolytics with non-users and ( ii ) three groups of anxiolytic users classified according to pattern ( frequency and regularity ) of use .
	manualset3
141480	3	408731	5	NULL	NULL	0	NULL	non-users	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The analyses compared ( i ) users of anxiolytics with non-users and ( ii ) three groups of anxiolytic users classified according to pattern ( frequency and regularity ) of use .
	manualset3
141481	4	408731	5	NULL	NULL	0	NULL	three groups	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The analyses compared ( i ) users of anxiolytics with non-users and ( ii ) three groups of anxiolytic users classified according to pattern ( frequency and regularity ) of use .
	manualset3
141482	5	408731	5	NULL	NULL	0	NULL	anxiolytic users	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The analyses compared ( i ) users of anxiolytics with non-users and ( ii ) three groups of anxiolytic users classified according to pattern ( frequency and regularity ) of use .
	manualset3
141483	6	408731	5	NULL	NULL	0	NULL	pattern 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The analyses compared ( i ) users of anxiolytics with non-users and ( ii ) three groups of anxiolytic users classified according to pattern ( frequency and regularity ) of use .
	manualset3
141484	7	408731	5	NULL	NULL	0	NULL	frequency 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The analyses compared ( i ) users of anxiolytics with non-users and ( ii ) three groups of anxiolytic users classified according to pattern ( frequency and regularity ) of use .
	manualset3
141485	8	408731	5	NULL	NULL	NULL	NULL	regularity 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The analyses compared ( i ) users of anxiolytics with non-users and ( ii ) three groups of anxiolytic users classified according to pattern ( frequency and regularity ) of use .
	manualset3
141486	9	408731	5	NULL	NULL	0	NULL	use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The analyses compared ( i ) users of anxiolytics with non-users and ( ii ) three groups of anxiolytic users classified according to pattern ( frequency and regularity ) of use .
	manualset3
144841	10	408731	5	NULL	NULL	0	NULL	analyses 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The analyses compared ( i ) users of anxiolytics with non-users and ( ii ) three groups of anxiolytic users classified according to pattern ( frequency and regularity ) of use .
	manualset3
141487	1	408732	5	NULL	NULL	0	NULL	analyses 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The analyses of sonochemically produced oxidants in the presence of various gases suggested that besides sonochemically formed hydrogen peroxide , nitrite and nitrate ions contributed to Fe ( II ) ion oxidation .
	manualset3
141488	2	408732	5	NULL	NULL	0	NULL	oxidants 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The analyses of sonochemically produced oxidants in the presence of various gases suggested that besides sonochemically formed hydrogen peroxide , nitrite and nitrate ions contributed to Fe ( II ) ion oxidation .
	manualset3
141489	3	408732	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The analyses of sonochemically produced oxidants in the presence of various gases suggested that besides sonochemically formed hydrogen peroxide , nitrite and nitrate ions contributed to Fe ( II ) ion oxidation .
	manualset3
141490	4	408732	5	NULL	NULL	0	NULL	gases 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The analyses of sonochemically produced oxidants in the presence of various gases suggested that besides sonochemically formed hydrogen peroxide , nitrite and nitrate ions contributed to Fe ( II ) ion oxidation .
	manualset3
141491	5	408732	5	NULL	NULL	NULL	NULL	hydrogen peroxide ions	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The analyses of sonochemically produced oxidants in the presence of various gases suggested that besides sonochemically formed hydrogen peroxide , nitrite and nitrate ions contributed to Fe ( II ) ion oxidation .
	manualset3
141492	6	408732	5	NULL	NULL	0	NULL	nitrite ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The analyses of sonochemically produced oxidants in the presence of various gases suggested that besides sonochemically formed hydrogen peroxide , nitrite and nitrate ions contributed to Fe ( II ) ion oxidation .
	manualset3
141493	7	408732	5	NULL	NULL	0	NULL	nitrate ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The analyses of sonochemically produced oxidants in the presence of various gases suggested that besides sonochemically formed hydrogen peroxide , nitrite and nitrate ions contributed to Fe ( II ) ion oxidation .
	manualset3
141494	8	408732	5	NULL	NULL	0	NULL	Fe ( II ) ion oxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The analyses of sonochemically produced oxidants in the presence of various gases suggested that besides sonochemically formed hydrogen peroxide , nitrite and nitrate ions contributed to Fe ( II ) ion oxidation .
	manualset3
141495	1	408733	5	NULL	NULL	0	NULL	analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of depth by this system provides for size constancy and , possibly , the calibration of relative motion .
	manualset3
141496	2	408733	5	NULL	NULL	0	NULL	depth 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of depth by this system provides for size constancy and , possibly , the calibration of relative motion .
	manualset3
141497	3	408733	5	NULL	NULL	0	NULL	system 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of depth by this system provides for size constancy and , possibly , the calibration of relative motion .
	manualset3
141498	4	408733	5	NULL	NULL	0	NULL	size constancy 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of depth by this system provides for size constancy and , possibly , the calibration of relative motion .
	manualset3
141499	5	408733	5	NULL	NULL	0	NULL	calibration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of depth by this system provides for size constancy and , possibly , the calibration of relative motion .
	manualset3
141500	6	408733	5	NULL	NULL	0	NULL	relative motion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of depth by this system provides for size constancy and , possibly , the calibration of relative motion .
	manualset3
141501	1	408734	5	NULL	NULL	0	NULL	analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of human operant behavior : A brief census of the literature : 1958-1981 .
	manualset3
141502	2	408734	5	NULL	NULL	0	NULL	human operant behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of human operant behavior : A brief census of the literature : 1958-1981 .
	manualset3
141503	3	408734	5	NULL	NULL	0	NULL	brief census	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of human operant behavior : A brief census of the literature : 1958-1981 .
	manualset3
141504	4	408734	5	NULL	NULL	0	NULL	literature 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of human operant behavior : A brief census of the literature : 1958-1981 .
	manualset3
141505	5	408734	5	NULL	NULL	0	NULL	1958-1981	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of human operant behavior : A brief census of the literature : 1958-1981 .
	manualset3
141506	1	408735	5	NULL	NULL	NULL	NULL	Chest pain 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Chest pain of esophageal origin in patients with a normal coronary angiogram and ergonovine-induced coronary spasm ) .
	manualset3
141507	2	408735	5	NULL	NULL	0	NULL	esophageal origin 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Chest pain of esophageal origin in patients with a normal coronary angiogram and ergonovine-induced coronary spasm ) .
	manualset3
141508	3	408735	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Chest pain of esophageal origin in patients with a normal coronary angiogram and ergonovine-induced coronary spasm ) .
	manualset3
141509	4	408735	5	NULL	NULL	0	NULL	normal coronary angiogram	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Chest pain of esophageal origin in patients with a normal coronary angiogram and ergonovine-induced coronary spasm ) .
	manualset3
141510	5	408735	5	NULL	NULL	0	NULL	ergonovine-induced coronary spasm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Chest pain of esophageal origin in patients with a normal coronary angiogram and ergonovine-induced coronary spasm ) .
	manualset3
141511	1	408736	5	NULL	NULL	0	NULL	blood lactate concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A rise in blood lactate concentrations was observed only at high doses of BM 13.677 , but was not related to an irreversible metabolic inhibition .
	manualset3
141512	2	408736	5	NULL	NULL	0	NULL	high doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A rise in blood lactate concentrations was observed only at high doses of BM 13.677 , but was not related to an irreversible metabolic inhibition .
	manualset3
141513	3	408736	5	NULL	NULL	0	NULL	 BM 13.677	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A rise in blood lactate concentrations was observed only at high doses of BM 13.677 , but was not related to an irreversible metabolic inhibition .
	manualset3
141514	4	408736	5	NULL	NULL	0	NULL	irreversible metabolic inhibition 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A rise in blood lactate concentrations was observed only at high doses of BM 13.677 , but was not related to an irreversible metabolic inhibition .
	manualset3
144842	5	408736	5	NULL	NULL	0	NULL	rise 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A rise in blood lactate concentrations was observed only at high doses of BM 13.677 , but was not related to an irreversible metabolic inhibition .
	manualset3
141515	1	408737	5	NULL	NULL	0	NULL	analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of isoniazid , sodium aminosalicylate and m-aminophenol ) .
	manualset3
141516	2	408737	5	NULL	NULL	0	NULL	isoniazid 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of isoniazid , sodium aminosalicylate and m-aminophenol ) .
	manualset3
141517	3	408737	5	NULL	NULL	0	NULL	sodium aminosalicylate	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of isoniazid , sodium aminosalicylate and m-aminophenol ) .
	manualset3
141518	4	408737	5	NULL	NULL	0	NULL	m-aminophenol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of isoniazid , sodium aminosalicylate and m-aminophenol ) .
	manualset3
141519	1	408738	5	NULL	NULL	0	NULL	analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of mortality in male subjects showed statistically significant excess of deaths from the circulatory system diseases ( SMR = 139 ) , in this from ischaemic heart disease ( SMR = 137 ) , cerebrovascular disease ( SMR = 188 ) and colon cancer ( SMR = 233 ) .
	manualset3
141520	2	408738	5	NULL	NULL	0	NULL	mortality 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of mortality in male subjects showed statistically significant excess of deaths from the circulatory system diseases ( SMR = 139 ) , in this from ischaemic heart disease ( SMR = 137 ) , cerebrovascular disease ( SMR = 188 ) and colon cancer ( SMR = 233 ) .
	manualset3
141521	3	408738	5	NULL	NULL	0	NULL	male subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of mortality in male subjects showed statistically significant excess of deaths from the circulatory system diseases ( SMR = 139 ) , in this from ischaemic heart disease ( SMR = 137 ) , cerebrovascular disease ( SMR = 188 ) and colon cancer ( SMR = 233 ) .
	manualset3
141522	4	408738	5	NULL	NULL	0	NULL	deaths 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of mortality in male subjects showed statistically significant excess of deaths from the circulatory system diseases ( SMR = 139 ) , in this from ischaemic heart disease ( SMR = 137 ) , cerebrovascular disease ( SMR = 188 ) and colon cancer ( SMR = 233 ) .
	manualset3
141523	5	408738	5	NULL	NULL	0	NULL	circulatory system diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of mortality in male subjects showed statistically significant excess of deaths from the circulatory system diseases ( SMR = 139 ) , in this from ischaemic heart disease ( SMR = 137 ) , cerebrovascular disease ( SMR = 188 ) and colon cancer ( SMR = 233 ) .
	manualset3
141524	6	408738	5	NULL	NULL	0	NULL	SMR = 139	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of mortality in male subjects showed statistically significant excess of deaths from the circulatory system diseases ( SMR = 139 ) , in this from ischaemic heart disease ( SMR = 137 ) , cerebrovascular disease ( SMR = 188 ) and colon cancer ( SMR = 233 ) .
	manualset3
141525	7	408738	5	NULL	NULL	0	NULL	ischaemic heart disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of mortality in male subjects showed statistically significant excess of deaths from the circulatory system diseases ( SMR = 139 ) , in this from ischaemic heart disease ( SMR = 137 ) , cerebrovascular disease ( SMR = 188 ) and colon cancer ( SMR = 233 ) .
	manualset3
141526	8	408738	5	NULL	NULL	0	NULL	SMR = 137	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of mortality in male subjects showed statistically significant excess of deaths from the circulatory system diseases ( SMR = 139 ) , in this from ischaemic heart disease ( SMR = 137 ) , cerebrovascular disease ( SMR = 188 ) and colon cancer ( SMR = 233 ) .
	manualset3
141527	9	408738	5	NULL	NULL	0	NULL	cerebrovascular disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of mortality in male subjects showed statistically significant excess of deaths from the circulatory system diseases ( SMR = 139 ) , in this from ischaemic heart disease ( SMR = 137 ) , cerebrovascular disease ( SMR = 188 ) and colon cancer ( SMR = 233 ) .
	manualset3
141528	10	408738	5	NULL	NULL	0	NULL	SMR = 188	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of mortality in male subjects showed statistically significant excess of deaths from the circulatory system diseases ( SMR = 139 ) , in this from ischaemic heart disease ( SMR = 137 ) , cerebrovascular disease ( SMR = 188 ) and colon cancer ( SMR = 233 ) .
	manualset3
141529	11	408738	5	NULL	NULL	0	NULL	colon cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of mortality in male subjects showed statistically significant excess of deaths from the circulatory system diseases ( SMR = 139 ) , in this from ischaemic heart disease ( SMR = 137 ) , cerebrovascular disease ( SMR = 188 ) and colon cancer ( SMR = 233 ) .
	manualset3
141530	12	408738	5	NULL	NULL	0	NULL	SMR = 233	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of mortality in male subjects showed statistically significant excess of deaths from the circulatory system diseases ( SMR = 139 ) , in this from ischaemic heart disease ( SMR = 137 ) , cerebrovascular disease ( SMR = 188 ) and colon cancer ( SMR = 233 ) .
	manualset3
141531	1	408739	5	NULL	NULL	0	NULL	analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of peptide spectral counts enabled the assessment of growth temperature specific proteins .
	manualset3
141532	2	408739	5	NULL	NULL	0	NULL	peptide spectral counts 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of peptide spectral counts enabled the assessment of growth temperature specific proteins .
	manualset3
141533	3	408739	5	NULL	NULL	0	NULL	assessment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of peptide spectral counts enabled the assessment of growth temperature specific proteins .
	manualset3
141534	4	408739	5	NULL	NULL	0	NULL	growth temperature specific proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of peptide spectral counts enabled the assessment of growth temperature specific proteins .
	manualset3
141535	1	408740	5	NULL	NULL	0	NULL	analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of the distributions of a local structural index indicates that the water molecules proximal to the graphene layer are considerably more structured than the rest and , thus , than the bulk .
	manualset3
141536	2	408740	5	NULL	NULL	0	NULL	distributions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of the distributions of a local structural index indicates that the water molecules proximal to the graphene layer are considerably more structured than the rest and , thus , than the bulk .
	manualset3
141537	3	408740	5	NULL	NULL	0	NULL	local structural index	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of the distributions of a local structural index indicates that the water molecules proximal to the graphene layer are considerably more structured than the rest and , thus , than the bulk .
	manualset3
141538	4	408740	5	NULL	NULL	0	NULL	water molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of the distributions of a local structural index indicates that the water molecules proximal to the graphene layer are considerably more structured than the rest and , thus , than the bulk .
	manualset3
141539	5	408740	5	NULL	NULL	0	NULL	graphene layer 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of the distributions of a local structural index indicates that the water molecules proximal to the graphene layer are considerably more structured than the rest and , thus , than the bulk .
	manualset3
141540	6	408740	5	NULL	NULL	0	NULL	bulk 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of the distributions of a local structural index indicates that the water molecules proximal to the graphene layer are considerably more structured than the rest and , thus , than the bulk .
	manualset3
141541	1	408741	5	NULL	NULL	0	NULL	analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of the system shows that the pedagogic aims followed by LTP are reached .
	manualset3
141542	2	408741	5	NULL	NULL	0	NULL	system 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of the system shows that the pedagogic aims followed by LTP are reached .
	manualset3
141543	3	408741	5	NULL	NULL	0	NULL	pedagogic aims 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of the system shows that the pedagogic aims followed by LTP are reached .
	manualset3
141544	4	408741	5	NULL	NULL	0	NULL	LTP 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The analysis of the system shows that the pedagogic aims followed by LTP are reached .
	manualset3
141545	1	408742	5	NULL	NULL	0	NULL	analyzed sample 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The analyzed sample was 352 total IgE values obtained by means of RIA in 611 patients of both sexes and ages from 5 to 15 years ( corrected ) , and the RAST results of every one of them .
	manualset3
141546	2	408742	5	NULL	NULL	0	NULL	352 total IgE values	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The analyzed sample was 352 total IgE values obtained by means of RIA in 611 patients of both sexes and ages from 5 to 15 years ( corrected ) , and the RAST results of every one of them .
	manualset3
141547	3	408742	5	NULL	NULL	0	NULL	RIA 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The analyzed sample was 352 total IgE values obtained by means of RIA in 611 patients of both sexes and ages from 5 to 15 years ( corrected ) , and the RAST results of every one of them .
	manualset3
141548	4	408742	5	NULL	NULL	0	NULL	611 patients	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The analyzed sample was 352 total IgE values obtained by means of RIA in 611 patients of both sexes and ages from 5 to 15 years ( corrected ) , and the RAST results of every one of them .
	manualset3
141549	5	408742	5	NULL	NULL	0	NULL	sexes 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The analyzed sample was 352 total IgE values obtained by means of RIA in 611 patients of both sexes and ages from 5 to 15 years ( corrected ) , and the RAST results of every one of them .
	manualset3
141550	6	408742	5	NULL	NULL	0	NULL	ages 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The analyzed sample was 352 total IgE values obtained by means of RIA in 611 patients of both sexes and ages from 5 to 15 years ( corrected ) , and the RAST results of every one of them .
	manualset3
141551	7	408742	5	NULL	NULL	0	NULL	5 to 15 years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The analyzed sample was 352 total IgE values obtained by means of RIA in 611 patients of both sexes and ages from 5 to 15 years ( corrected ) , and the RAST results of every one of them .
	manualset3
141552	8	408742	5	NULL	NULL	0	NULL	RAST results	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The analyzed sample was 352 total IgE values obtained by means of RIA in 611 patients of both sexes and ages from 5 to 15 years ( corrected ) , and the RAST results of every one of them .
	manualset3
144843	9	408742	5	NULL	NULL	0	NULL	one 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The analyzed sample was 352 total IgE values obtained by means of RIA in 611 patients of both sexes and ages from 5 to 15 years ( corrected ) , and the RAST results of every one of them .
	manualset3
141553	1	408743	5	NULL	NULL	0	NULL	erythropoietic activity production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A rise in erythropoietic activity production by bone marrow cells testified that elevation of hemopoiesis inducing microenvironment function is the base of stimulating effect of N-ANA on hemopoiesis .
	manualset3
141554	2	408743	5	NULL	NULL	0	NULL	bone marrow cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A rise in erythropoietic activity production by bone marrow cells testified that elevation of hemopoiesis inducing microenvironment function is the base of stimulating effect of N-ANA on hemopoiesis .
	manualset3
141555	3	408743	5	NULL	NULL	0	NULL	elevation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A rise in erythropoietic activity production by bone marrow cells testified that elevation of hemopoiesis inducing microenvironment function is the base of stimulating effect of N-ANA on hemopoiesis .
	manualset3
141556	4	408743	5	NULL	NULL	0	NULL	hemopoiesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A rise in erythropoietic activity production by bone marrow cells testified that elevation of hemopoiesis inducing microenvironment function is the base of stimulating effect of N-ANA on hemopoiesis .
	manualset3
141557	5	408743	5	NULL	NULL	0	NULL	microenvironment function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A rise in erythropoietic activity production by bone marrow cells testified that elevation of hemopoiesis inducing microenvironment function is the base of stimulating effect of N-ANA on hemopoiesis .
	manualset3
141558	6	408743	5	NULL	NULL	0	NULL	 stimulating effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A rise in erythropoietic activity production by bone marrow cells testified that elevation of hemopoiesis inducing microenvironment function is the base of stimulating effect of N-ANA on hemopoiesis .
	manualset3
141559	7	408743	5	NULL	NULL	0	NULL	N-ANA	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A rise in erythropoietic activity production by bone marrow cells testified that elevation of hemopoiesis inducing microenvironment function is the base of stimulating effect of N-ANA on hemopoiesis .
	manualset3
141560	8	408743	5	NULL	NULL	0	NULL	hemopoiesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A rise in erythropoietic activity production by bone marrow cells testified that elevation of hemopoiesis inducing microenvironment function is the base of stimulating effect of N-ANA on hemopoiesis .
	manualset3
141561	1	408744	5	NULL	NULL	0	NULL	anastomosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The anastomosis seemed to be associated with hypoplasia of the right vertebral artery .
	manualset3
141562	2	408744	5	NULL	NULL	0	NULL	hypoplasia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The anastomosis seemed to be associated with hypoplasia of the right vertebral artery .
	manualset3
141563	3	408744	5	NULL	NULL	0	NULL	right vertebral artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The anastomosis seemed to be associated with hypoplasia of the right vertebral artery .
	manualset3
141564	1	408745	5	NULL	NULL	0	NULL	anatomical distribution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The anatomical distribution of mercaptopurine was investigated in rats at dose levels of 2.5 and 25 mg/kg iv .
	manualset3
141565	2	408745	5	NULL	NULL	0	NULL	mercaptopurine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The anatomical distribution of mercaptopurine was investigated in rats at dose levels of 2.5 and 25 mg/kg iv .
	manualset3
141566	3	408745	5	NULL	NULL	0	NULL	rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The anatomical distribution of mercaptopurine was investigated in rats at dose levels of 2.5 and 25 mg/kg iv .
	manualset3
141567	4	408745	5	NULL	NULL	0	NULL	dose levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The anatomical distribution of mercaptopurine was investigated in rats at dose levels of 2.5 and 25 mg/kg iv .
	manualset3
141568	5	408745	5	NULL	NULL	0	NULL	2.5 mg/kg iv	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The anatomical distribution of mercaptopurine was investigated in rats at dose levels of 2.5 and 25 mg/kg iv .
	manualset3
141569	6	408745	5	NULL	NULL	0	NULL	25 mg/kg iv	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The anatomical distribution of mercaptopurine was investigated in rats at dose levels of 2.5 and 25 mg/kg iv .
	manualset3
141570	1	408746	5	NULL	NULL	0	NULL	androgen-producing activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The androgen-producing activity appeared on day 9 after birth ( 1.16 + / - 0.25 pmol/2 ovaries/48 h ) , when follicles with more than two layers of granulosa cells developed .
	manualset3
141571	2	408746	5	NULL	NULL	0	NULL	day 9 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	The androgen-producing activity appeared on day 9 after birth ( 1.16 + / - 0.25 pmol/2 ovaries/48 h ) , when follicles with more than two layers of granulosa cells developed .
	manualset3
141572	3	408746	5	NULL	NULL	0	NULL	birth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The androgen-producing activity appeared on day 9 after birth ( 1.16 + / - 0.25 pmol/2 ovaries/48 h ) , when follicles with more than two layers of granulosa cells developed .
	manualset3
141573	4	408746	5	NULL	NULL	0	NULL	 1.16 + / - 0.25 pmol/2 ovaries/48 h	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The androgen-producing activity appeared on day 9 after birth ( 1.16 + / - 0.25 pmol/2 ovaries/48 h ) , when follicles with more than two layers of granulosa cells developed .
	manualset3
141574	5	408746	5	NULL	NULL	0	NULL	follicles 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The androgen-producing activity appeared on day 9 after birth ( 1.16 + / - 0.25 pmol/2 ovaries/48 h ) , when follicles with more than two layers of granulosa cells developed .
	manualset3
141575	6	408746	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The androgen-producing activity appeared on day 9 after birth ( 1.16 + / - 0.25 pmol/2 ovaries/48 h ) , when follicles with more than two layers of granulosa cells developed .
	manualset3
141576	7	408746	5	NULL	NULL	0	NULL	layers of granulosa cells	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The androgen-producing activity appeared on day 9 after birth ( 1.16 + / - 0.25 pmol/2 ovaries/48 h ) , when follicles with more than two layers of granulosa cells developed .
	manualset3
141577	1	408747	5	NULL	NULL	0	NULL	aneurysm 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aneurysm was resected and the vein repaired by direct suture .
	manualset3
141578	2	408747	5	NULL	NULL	0	NULL	vein 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The aneurysm was resected and the vein repaired by direct suture .
	manualset3
141579	3	408747	5	NULL	NULL	0	NULL	direct suture 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aneurysm was resected and the vein repaired by direct suture .
	manualset3
141580	1	408748	5	NULL	NULL	0	NULL	angle 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The angle is 9.42 degrees + / - 4.1 degrees in the population of this country .
	manualset3
141581	2	408748	5	NULL	NULL	0	NULL	9.42 degrees + / - 4.1 degrees	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The angle is 9.42 degrees + / - 4.1 degrees in the population of this country .
	manualset3
141582	3	408748	5	NULL	NULL	0	NULL	population 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The angle is 9.42 degrees + / - 4.1 degrees in the population of this country .
	manualset3
141583	4	408748	5	NULL	NULL	0	NULL	country 	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The angle is 9.42 degrees + / - 4.1 degrees in the population of this country .
	manualset3
141584	1	408749	5	NULL	NULL	0	NULL	animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The animals were divided into three groups according to neurological symptoms : sham-operation group , group A ( hemiparesis only ) , and group B ( hemiparesis with unconsciousness ) .
	manualset3
141585	2	408749	5	NULL	NULL	0	NULL	three groups	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The animals were divided into three groups according to neurological symptoms : sham-operation group , group A ( hemiparesis only ) , and group B ( hemiparesis with unconsciousness ) .
	manualset3
141586	3	408749	5	NULL	NULL	0	NULL	neurological symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The animals were divided into three groups according to neurological symptoms : sham-operation group , group A ( hemiparesis only ) , and group B ( hemiparesis with unconsciousness ) .
	manualset3
141587	4	408749	5	NULL	NULL	0	NULL	sham-operation group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The animals were divided into three groups according to neurological symptoms : sham-operation group , group A ( hemiparesis only ) , and group B ( hemiparesis with unconsciousness ) .
	manualset3
141588	5	408749	5	NULL	NULL	0	NULL	group A ( hemiparesis only )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The animals were divided into three groups according to neurological symptoms : sham-operation group , group A ( hemiparesis only ) , and group B ( hemiparesis with unconsciousness ) .
	manualset3
141589	6	408749	5	NULL	NULL	0	NULL	group B ( hemiparesis with unconsciousness )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The animals were divided into three groups according to neurological symptoms : sham-operation group , group A ( hemiparesis only ) , and group B ( hemiparesis with unconsciousness ) .
	manualset3
141590	1	408750	5	NULL	NULL	0	NULL	rivastigmine patch	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A rivastigmine patch for dementia .
	manualset3
141591	2	408750	5	NULL	NULL	0	NULL	dementia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A rivastigmine patch for dementia .
	manualset3
141592	1	408751	5	NULL	NULL	0	NULL	animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The animals were fed a low protein diet ( 94 g CP/kg DM and 11 MJ ME/kg DM ) .
	manualset3
141593	2	408751	5	NULL	NULL	0	NULL	low protein diet 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The animals were fed a low protein diet ( 94 g CP/kg DM and 11 MJ ME/kg DM ) .
	manualset3
141594	3	408751	5	NULL	NULL	0	NULL	94 g CP/kg DM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The animals were fed a low protein diet ( 94 g CP/kg DM and 11 MJ ME/kg DM ) .
	manualset3
141595	4	408751	5	NULL	NULL	0	NULL	11 MJ ME/kg DM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The animals were fed a low protein diet ( 94 g CP/kg DM and 11 MJ ME/kg DM ) .
	manualset3
141596	1	408752	5	NULL	NULL	0	NULL	ankle 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The ankle is a complex articular structure with contributions from the talocrural , subtalar , and inferior tibiofibular joints .
	manualset3
141597	2	408752	5	NULL	NULL	0	NULL	complex articular structure 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The ankle is a complex articular structure with contributions from the talocrural , subtalar , and inferior tibiofibular joints .
	manualset3
141598	3	408752	5	NULL	NULL	0	NULL	contributions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ankle is a complex articular structure with contributions from the talocrural , subtalar , and inferior tibiofibular joints .
	manualset3
141599	4	408752	5	NULL	NULL	0	NULL	talocrural joints	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The ankle is a complex articular structure with contributions from the talocrural , subtalar , and inferior tibiofibular joints .
	manualset3
141600	5	408752	5	NULL	NULL	0	NULL	subtalar joints	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The ankle is a complex articular structure with contributions from the talocrural , subtalar , and inferior tibiofibular joints .
	manualset3
141601	6	408752	5	NULL	NULL	0	NULL	inferior tibiofibular joints	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The ankle is a complex articular structure with contributions from the talocrural , subtalar , and inferior tibiofibular joints .
	manualset3
141602	1	408753	5	NULL	NULL	0	NULL	annual growth rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The annual growth rate is 4.22 % .
	manualset3
141603	2	408753	5	NULL	NULL	0	NULL	4.22 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The annual growth rate is 4.22 % .
	manualset3
141604	1	408754	5	NULL	NULL	0	NULL	Sigma ( C15-C34 )	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The annual riverine input of Sigma ( C15-C34 ) from the PRD to the coastal ocean was 360 tons/year , or the equivalent of approximately 8 , 800 tons/year of petroleum hydrocarbons .
	manualset3
141605	2	408754	5	NULL	NULL	0	NULL	PRD 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The annual riverine input of Sigma ( C15-C34 ) from the PRD to the coastal ocean was 360 tons/year , or the equivalent of approximately 8 , 800 tons/year of petroleum hydrocarbons .
	manualset3
141606	3	408754	5	NULL	NULL	0	NULL	coastal ocean	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The annual riverine input of Sigma ( C15-C34 ) from the PRD to the coastal ocean was 360 tons/year , or the equivalent of approximately 8 , 800 tons/year of petroleum hydrocarbons .
	manualset3
141607	4	408754	5	NULL	NULL	0	NULL	360 tons/year	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The annual riverine input of Sigma ( C15-C34 ) from the PRD to the coastal ocean was 360 tons/year , or the equivalent of approximately 8 , 800 tons/year of petroleum hydrocarbons .
	manualset3
141608	5	408754	5	NULL	NULL	0	NULL	equivalent 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The annual riverine input of Sigma ( C15-C34 ) from the PRD to the coastal ocean was 360 tons/year , or the equivalent of approximately 8 , 800 tons/year of petroleum hydrocarbons .
	manualset3
141609	6	408754	5	NULL	NULL	0	NULL	8 , 800 tons/year	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The annual riverine input of Sigma ( C15-C34 ) from the PRD to the coastal ocean was 360 tons/year , or the equivalent of approximately 8 , 800 tons/year of petroleum hydrocarbons .
	manualset3
141610	7	408754	5	NULL	NULL	0	NULL	petroleum hydrocarbons 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The annual riverine input of Sigma ( C15-C34 ) from the PRD to the coastal ocean was 360 tons/year , or the equivalent of approximately 8 , 800 tons/year of petroleum hydrocarbons .
	manualset3
141611	1	408755	5	NULL	NULL	0	NULL	annulus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The annulus and adjacent longitudinal ligaments were also analyzed histologically .
	manualset3
141612	2	408755	5	NULL	NULL	0	NULL	adjacent longitudinal ligaments	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The annulus and adjacent longitudinal ligaments were also analyzed histologically .
	manualset3
141613	1	408756	5	NULL	NULL	0	NULL	anorectic activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The anorectic activity of calcitonin was destroyed by exposing the hormone to heat , trypsin , or hydrogen peroxide .
	manualset3
141614	2	408756	5	NULL	NULL	0	NULL	calcitonin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The anorectic activity of calcitonin was destroyed by exposing the hormone to heat , trypsin , or hydrogen peroxide .
	manualset3
141615	3	408756	5	NULL	NULL	0	NULL	hormone 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The anorectic activity of calcitonin was destroyed by exposing the hormone to heat , trypsin , or hydrogen peroxide .
	manualset3
141616	4	408756	5	NULL	NULL	0	NULL	heat 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The anorectic activity of calcitonin was destroyed by exposing the hormone to heat , trypsin , or hydrogen peroxide .
	manualset3
141617	5	408756	5	NULL	NULL	0	NULL	trypsin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The anorectic activity of calcitonin was destroyed by exposing the hormone to heat , trypsin , or hydrogen peroxide .
	manualset3
141618	6	408756	5	NULL	NULL	0	NULL	hydrogen peroxide	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The anorectic activity of calcitonin was destroyed by exposing the hormone to heat , trypsin , or hydrogen peroxide .
	manualset3
141619	1	408757	5	NULL	NULL	0	NULL	antagonism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The antagonism of all investigated compounds for toward reserpine , first of all of the preparations III , IV , V and IX , indicates an antidepressive activity dependent on a stimulation of the adrenergic system .
	manualset3
141620	2	408757	5	NULL	NULL	0	NULL	investigated compounds 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The antagonism of all investigated compounds for toward reserpine , first of all of the preparations III , IV , V and IX , indicates an antidepressive activity dependent on a stimulation of the adrenergic system .
	manualset3
141621	3	408757	5	NULL	NULL	0	NULL	reserpine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The antagonism of all investigated compounds for toward reserpine , first of all of the preparations III , IV , V and IX , indicates an antidepressive activity dependent on a stimulation of the adrenergic system .
	manualset3
141622	4	408757	5	NULL	NULL	0	NULL	preparations III	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The antagonism of all investigated compounds for toward reserpine , first of all of the preparations III , IV , V and IX , indicates an antidepressive activity dependent on a stimulation of the adrenergic system .
	manualset3
141623	5	408757	5	NULL	NULL	0	NULL	preparations IV	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The antagonism of all investigated compounds for toward reserpine , first of all of the preparations III , IV , V and IX , indicates an antidepressive activity dependent on a stimulation of the adrenergic system .
	manualset3
141624	6	408757	5	NULL	NULL	0	NULL	preparations V	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The antagonism of all investigated compounds for toward reserpine , first of all of the preparations III , IV , V and IX , indicates an antidepressive activity dependent on a stimulation of the adrenergic system .
	manualset3
141625	7	408757	5	NULL	NULL	0	NULL	preparations IX	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The antagonism of all investigated compounds for toward reserpine , first of all of the preparations III , IV , V and IX , indicates an antidepressive activity dependent on a stimulation of the adrenergic system .
	manualset3
141626	8	408757	5	NULL	NULL	0	NULL	antidepressive activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The antagonism of all investigated compounds for toward reserpine , first of all of the preparations III , IV , V and IX , indicates an antidepressive activity dependent on a stimulation of the adrenergic system .
	manualset3
141627	9	408757	5	NULL	NULL	0	NULL	stimulation of the adrenergic system	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The antagonism of all investigated compounds for toward reserpine , first of all of the preparations III , IV , V and IX , indicates an antidepressive activity dependent on a stimulation of the adrenergic system .
	manualset3
141628	1	408758	5	NULL	NULL	0	NULL	robustness test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A robustness test is successfully performed using distorted SPM images .
	manualset3
141629	2	408758	5	NULL	NULL	0	NULL	distorted SPM images	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A robustness test is successfully performed using distorted SPM images .
	manualset3
141630	1	408759	5	NULL	NULL	0	NULL	anterior stand-alone approach ( ASAA )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The anterior stand-alone approach ( ASAA ) during the acute phase of spondylodiscitis : results in 40 consecutively treated patients .
	manualset3
141632	2	408759	5	NULL	NULL	0	NULL	acute phase of spondylodiscitis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The anterior stand-alone approach ( ASAA ) during the acute phase of spondylodiscitis : results in 40 consecutively treated patients .
	manualset3
141633	3	408759	5	NULL	NULL	0	NULL	results 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The anterior stand-alone approach ( ASAA ) during the acute phase of spondylodiscitis : results in 40 consecutively treated patients .
	manualset3
141634	4	408759	5	NULL	NULL	0	NULL	 40 consecutively treated patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The anterior stand-alone approach ( ASAA ) during the acute phase of spondylodiscitis : results in 40 consecutively treated patients .
	manualset3
141635	1	408760	5	NULL	NULL	NULL	NULL	anthropourgic foci 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The anthropourgic foci of leptospirosis caused by L. pomona are of the leading epidemiological importance .
	manualset3
141636	2	408760	5	NULL	NULL	0	NULL	leptospirosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The anthropourgic foci of leptospirosis caused by L. pomona are of the leading epidemiological importance .
	manualset3
141637	3	408760	5	NULL	NULL	0	NULL	L. pomona	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The anthropourgic foci of leptospirosis caused by L. pomona are of the leading epidemiological importance .
	manualset3
141638	4	408760	5	NULL	NULL	NULL	NULL	epidemiological importance 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The anthropourgic foci of leptospirosis caused by L. pomona are of the leading epidemiological importance .
	manualset3
141639	1	408761	5	NULL	NULL	0	NULL	anti-CMV activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-CMV activity of CRDS in this study , therefore , had a p value & lt ; 0.001 , based on these historical controls .
	manualset3
141640	2	408761	5	NULL	NULL	0	NULL	CRDS 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-CMV activity of CRDS in this study , therefore , had a p value & lt ; 0.001 , based on these historical controls .
	manualset3
141641	3	408761	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-CMV activity of CRDS in this study , therefore , had a p value & lt ; 0.001 , based on these historical controls .
	manualset3
141642	4	408761	5	NULL	NULL	0	NULL	p value & lt ; 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-CMV activity of CRDS in this study , therefore , had a p value & lt ; 0.001 , based on these historical controls .
	manualset3
141643	5	408761	5	NULL	NULL	0	NULL	controls 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-CMV activity of CRDS in this study , therefore , had a p value & lt ; 0.001 , based on these historical controls .
	manualset3
141644	1	408762	5	NULL	NULL	0	NULL	anti-NB1 antibodies 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-NB1 antibodies can be specifically removed from normal mouse sera by absorption of the sera with homogenized brain tissue of mouse , rat , guinea pig , chicken , and man and by homogenized kidney tissue of mouse and man .
	manualset3
141645	2	408762	5	NULL	NULL	0	NULL	normal mouse sera	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-NB1 antibodies can be specifically removed from normal mouse sera by absorption of the sera with homogenized brain tissue of mouse , rat , guinea pig , chicken , and man and by homogenized kidney tissue of mouse and man .
	manualset3
141646	3	408762	5	NULL	NULL	0	NULL	absorption 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-NB1 antibodies can be specifically removed from normal mouse sera by absorption of the sera with homogenized brain tissue of mouse , rat , guinea pig , chicken , and man and by homogenized kidney tissue of mouse and man .
	manualset3
141647	4	408762	5	NULL	NULL	0	NULL	sera 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-NB1 antibodies can be specifically removed from normal mouse sera by absorption of the sera with homogenized brain tissue of mouse , rat , guinea pig , chicken , and man and by homogenized kidney tissue of mouse and man .
	manualset3
141648	5	408762	5	NULL	NULL	0	NULL	homogenized brain tissue 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-NB1 antibodies can be specifically removed from normal mouse sera by absorption of the sera with homogenized brain tissue of mouse , rat , guinea pig , chicken , and man and by homogenized kidney tissue of mouse and man .
	manualset3
141649	6	408762	5	NULL	NULL	0	NULL	mouse 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-NB1 antibodies can be specifically removed from normal mouse sera by absorption of the sera with homogenized brain tissue of mouse , rat , guinea pig , chicken , and man and by homogenized kidney tissue of mouse and man .
	manualset3
141650	7	408762	5	NULL	NULL	0	NULL	rat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-NB1 antibodies can be specifically removed from normal mouse sera by absorption of the sera with homogenized brain tissue of mouse , rat , guinea pig , chicken , and man and by homogenized kidney tissue of mouse and man .
	manualset3
141651	8	408762	5	NULL	NULL	0	NULL	guinea pig	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-NB1 antibodies can be specifically removed from normal mouse sera by absorption of the sera with homogenized brain tissue of mouse , rat , guinea pig , chicken , and man and by homogenized kidney tissue of mouse and man .
	manualset3
141652	9	408762	5	NULL	NULL	0	NULL	chicken 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-NB1 antibodies can be specifically removed from normal mouse sera by absorption of the sera with homogenized brain tissue of mouse , rat , guinea pig , chicken , and man and by homogenized kidney tissue of mouse and man .
	manualset3
141653	10	408762	5	NULL	NULL	0	NULL	man 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-NB1 antibodies can be specifically removed from normal mouse sera by absorption of the sera with homogenized brain tissue of mouse , rat , guinea pig , chicken , and man and by homogenized kidney tissue of mouse and man .
	manualset3
141654	11	408762	5	NULL	NULL	0	NULL	homogenized kidney tissue 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-NB1 antibodies can be specifically removed from normal mouse sera by absorption of the sera with homogenized brain tissue of mouse , rat , guinea pig , chicken , and man and by homogenized kidney tissue of mouse and man .
	manualset3
141655	12	408762	5	NULL	NULL	0	NULL	mouse 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-NB1 antibodies can be specifically removed from normal mouse sera by absorption of the sera with homogenized brain tissue of mouse , rat , guinea pig , chicken , and man and by homogenized kidney tissue of mouse and man .
	manualset3
141656	13	408762	5	NULL	NULL	0	NULL	man 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-NB1 antibodies can be specifically removed from normal mouse sera by absorption of the sera with homogenized brain tissue of mouse , rat , guinea pig , chicken , and man and by homogenized kidney tissue of mouse and man .
	manualset3
141657	1	408763	5	NULL	NULL	0	NULL	anti-hCGbeta antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-hCGbeta antibody was used to identify the fusion protein .
	manualset3
141658	2	408763	5	NULL	NULL	0	NULL	fusion protein	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-hCGbeta antibody was used to identify the fusion protein .
	manualset3
141659	1	408764	5	NULL	NULL	0	NULL	anti-inflammatory activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-inflammatory activity of the IL-1 receptor antagonist , IL-1ra , was evaluated in the acetic acid ( HOAc ) - induced model of colitis in rats .
	manualset3
141660	2	408764	5	NULL	NULL	0	NULL	IL-1 receptor antagonist , IL-1ra	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-inflammatory activity of the IL-1 receptor antagonist , IL-1ra , was evaluated in the acetic acid ( HOAc ) - induced model of colitis in rats .
	manualset3
141661	3	408764	5	NULL	NULL	0	NULL	 acetic acid ( HOAc ) - induced model of colitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-inflammatory activity of the IL-1 receptor antagonist , IL-1ra , was evaluated in the acetic acid ( HOAc ) - induced model of colitis in rats .
	manualset3
141662	4	408764	5	NULL	NULL	0	NULL	rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-inflammatory activity of the IL-1 receptor antagonist , IL-1ra , was evaluated in the acetic acid ( HOAc ) - induced model of colitis in rats .
	manualset3
141663	1	408765	5	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A role for NF-kappa B activation in perforin expression of NK cells upon IL-2 receptor signaling .
	manualset3
141664	2	408765	5	NULL	NULL	0	NULL	NF-kappa B activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A role for NF-kappa B activation in perforin expression of NK cells upon IL-2 receptor signaling .
	manualset3
141665	3	408765	5	NULL	NULL	0	NULL	perforin expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A role for NF-kappa B activation in perforin expression of NK cells upon IL-2 receptor signaling .
	manualset3
141666	4	408765	5	NULL	NULL	0	NULL	NK cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A role for NF-kappa B activation in perforin expression of NK cells upon IL-2 receptor signaling .
	manualset3
141667	5	408765	5	NULL	NULL	0	NULL	IL-2 receptor signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A role for NF-kappa B activation in perforin expression of NK cells upon IL-2 receptor signaling .
	manualset3
141668	1	408766	5	NULL	NULL	0	NULL	anti-inflammatory activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-inflammatory activity was evidenced by decreased carrageenan-induced rat paw edema and PGE elevation .
	manualset3
141669	2	408766	5	NULL	NULL	0	NULL	carrageenan-induced rat paw edema	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-inflammatory activity was evidenced by decreased carrageenan-induced rat paw edema and PGE elevation .
	manualset3
141670	3	408766	5	NULL	NULL	0	NULL	PGE elevation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-inflammatory activity was evidenced by decreased carrageenan-induced rat paw edema and PGE elevation .
	manualset3
141671	1	408767	5	NULL	NULL	0	NULL	anti-inflammatory glucocorticoid dexamethasone	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-inflammatory glucocorticoid dexamethasone selectively blocked LPS-stimulated IL-6 mRNA accumulation but not TNF-alpha .
	manualset3
141672	2	408767	5	NULL	NULL	0	NULL	LPS-stimulated IL-6 mRNA accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-inflammatory glucocorticoid dexamethasone selectively blocked LPS-stimulated IL-6 mRNA accumulation but not TNF-alpha .
	manualset3
141673	3	408767	5	NULL	NULL	0	NULL	TNF-alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-inflammatory glucocorticoid dexamethasone selectively blocked LPS-stimulated IL-6 mRNA accumulation but not TNF-alpha .
	manualset3
141674	1	408768	5	NULL	NULL	0	NULL	anti-proliferative effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-proliferative effect of inhibitor of telomerase on cultured retinal pigment epithelial cells .
	manualset3
141675	2	408768	5	NULL	NULL	0	NULL	inhibitor of telomerase	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-proliferative effect of inhibitor of telomerase on cultured retinal pigment epithelial cells .
	manualset3
141676	3	408768	5	NULL	NULL	0	NULL	cultured retinal pigment epithelial cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The anti-proliferative effect of inhibitor of telomerase on cultured retinal pigment epithelial cells .
	manualset3
141677	1	408769	5	NULL	NULL	0	NULL	antibacterial potency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The antibacterial potency of 250 mg/kg of amikacin is comparable to that of 100 mg/kg of hydroxygentamicin .
	manualset3
141678	2	408769	5	NULL	NULL	0	NULL	250 mg/kg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The antibacterial potency of 250 mg/kg of amikacin is comparable to that of 100 mg/kg of hydroxygentamicin .
	manualset3
141679	3	408769	5	NULL	NULL	0	NULL	amikacin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The antibacterial potency of 250 mg/kg of amikacin is comparable to that of 100 mg/kg of hydroxygentamicin .
	manualset3
141680	4	408769	5	NULL	NULL	0	NULL	100 mg/kg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The antibacterial potency of 250 mg/kg of amikacin is comparable to that of 100 mg/kg of hydroxygentamicin .
	manualset3
141681	5	408769	5	NULL	NULL	0	NULL	hydroxygentamicin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The antibacterial potency of 250 mg/kg of amikacin is comparable to that of 100 mg/kg of hydroxygentamicin .
	manualset3
141682	1	408770	5	NULL	NULL	0	NULL	antibodies 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The antibodies were unable to induce the biochemical changes in the zona associated with the postfertilization block to polyspermy and had no detectable effect on preimplantation development .
	manualset3
141683	2	408770	5	NULL	NULL	0	NULL	biochemical changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The antibodies were unable to induce the biochemical changes in the zona associated with the postfertilization block to polyspermy and had no detectable effect on preimplantation development .
	manualset3
141684	3	408770	5	NULL	NULL	0	NULL	zona 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The antibodies were unable to induce the biochemical changes in the zona associated with the postfertilization block to polyspermy and had no detectable effect on preimplantation development .
	manualset3
141685	4	408770	5	NULL	NULL	0	NULL	postfertilization block 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The antibodies were unable to induce the biochemical changes in the zona associated with the postfertilization block to polyspermy and had no detectable effect on preimplantation development .
	manualset3
141686	5	408770	5	NULL	NULL	0	NULL	polyspermy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The antibodies were unable to induce the biochemical changes in the zona associated with the postfertilization block to polyspermy and had no detectable effect on preimplantation development .
	manualset3
141687	6	408770	5	NULL	NULL	0	NULL	effect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The antibodies were unable to induce the biochemical changes in the zona associated with the postfertilization block to polyspermy and had no detectable effect on preimplantation development .
	manualset3
141688	7	408770	5	NULL	NULL	0	NULL	preimplantation development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The antibodies were unable to induce the biochemical changes in the zona associated with the postfertilization block to polyspermy and had no detectable effect on preimplantation development .
	manualset3
141689	1	408771	5	NULL	NULL	0	NULL	antigen 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The antigen isolated either from testis or sperm showed mainly the same spots .
	manualset3
141690	2	408771	5	NULL	NULL	0	NULL	testis 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The antigen isolated either from testis or sperm showed mainly the same spots .
	manualset3
141691	3	408771	5	NULL	NULL	0	NULL	sperm 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The antigen isolated either from testis or sperm showed mainly the same spots .
	manualset3
141692	4	408771	5	NULL	NULL	0	NULL	same spots	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The antigen isolated either from testis or sperm showed mainly the same spots .
	manualset3
141693	1	408772	5	NULL	NULL	0	NULL	antigenic structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The antigenic structure of the Central Asian variants and the Burmese types of HEV was found similar .
	manualset3
141694	2	408772	5	NULL	NULL	0	NULL	Central Asian variants	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The antigenic structure of the Central Asian variants and the Burmese types of HEV was found similar .
	manualset3
141695	3	408772	5	NULL	NULL	0	NULL	Burmese types of HEV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The antigenic structure of the Central Asian variants and the Burmese types of HEV was found similar .
	manualset3
141696	1	408773	5	NULL	NULL	0	NULL	antigenic targets	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The antigenic targets for alloantibodies formed after leucocyte transfusions and multiple allogeneic pregnancies were defined by the EA rosette inhibition ( EAI ) assay in several congenic and recombinant inbred rat strains .
	manualset3
141697	2	408773	5	NULL	NULL	0	NULL	alloantibodies 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The antigenic targets for alloantibodies formed after leucocyte transfusions and multiple allogeneic pregnancies were defined by the EA rosette inhibition ( EAI ) assay in several congenic and recombinant inbred rat strains .
	manualset3
141698	3	408773	5	NULL	NULL	NULL	NULL	leucocyte transfusions	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The antigenic targets for alloantibodies formed after leucocyte transfusions and multiple allogeneic pregnancies were defined by the EA rosette inhibition ( EAI ) assay in several congenic and recombinant inbred rat strains .
	manualset3
141699	4	408773	5	NULL	NULL	0	NULL	multiple allogeneic pregnancies 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The antigenic targets for alloantibodies formed after leucocyte transfusions and multiple allogeneic pregnancies were defined by the EA rosette inhibition ( EAI ) assay in several congenic and recombinant inbred rat strains .
	manualset3
141700	5	408773	5	NULL	NULL	0	NULL	EA rosette inhibition ( EAI ) assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The antigenic targets for alloantibodies formed after leucocyte transfusions and multiple allogeneic pregnancies were defined by the EA rosette inhibition ( EAI ) assay in several congenic and recombinant inbred rat strains .
	manualset3
141701	6	408773	5	NULL	NULL	0	NULL	congenic inbred rat strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The antigenic targets for alloantibodies formed after leucocyte transfusions and multiple allogeneic pregnancies were defined by the EA rosette inhibition ( EAI ) assay in several congenic and recombinant inbred rat strains .
	manualset3
141702	7	408773	5	NULL	NULL	0	NULL	recombinant inbred rat strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The antigenic targets for alloantibodies formed after leucocyte transfusions and multiple allogeneic pregnancies were defined by the EA rosette inhibition ( EAI ) assay in several congenic and recombinant inbred rat strains .
	manualset3
141703	1	408774	5	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A role for PKC activation had been noted in several renal diseases , but two that have had most investigation are diabetic nephropathy and kidney cancer .
	manualset3
141704	2	408774	5	NULL	NULL	0	NULL	PKC activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A role for PKC activation had been noted in several renal diseases , but two that have had most investigation are diabetic nephropathy and kidney cancer .
	manualset3
141705	3	408774	5	NULL	NULL	0	NULL	several renal diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A role for PKC activation had been noted in several renal diseases , but two that have had most investigation are diabetic nephropathy and kidney cancer .
	manualset3
141706	4	408774	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A role for PKC activation had been noted in several renal diseases , but two that have had most investigation are diabetic nephropathy and kidney cancer .
	manualset3
141707	5	408774	5	NULL	NULL	0	NULL	diabetic nephropathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A role for PKC activation had been noted in several renal diseases , but two that have had most investigation are diabetic nephropathy and kidney cancer .
	manualset3
141708	6	408774	5	NULL	NULL	0	NULL	kidney cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A role for PKC activation had been noted in several renal diseases , but two that have had most investigation are diabetic nephropathy and kidney cancer .
	manualset3
142567	7	408774	5	NULL	NULL	0	NULL	investigation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A role for PKC activation had been noted in several renal diseases , but two that have had most investigation are diabetic nephropathy and kidney cancer .
	manualset3
141709	1	408775	5	NULL	NULL	0	NULL	antigens 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The antigens of the Drh system appear to be the most strongly immunogenic , and are thus of greatest importance for the experimental use of these animals , such as in transplantation and blood transfusion .
	manualset3
141710	2	408775	5	NULL	NULL	0	NULL	Drh system	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The antigens of the Drh system appear to be the most strongly immunogenic , and are thus of greatest importance for the experimental use of these animals , such as in transplantation and blood transfusion .
	manualset3
141711	3	408775	5	NULL	NULL	0	NULL	importance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The antigens of the Drh system appear to be the most strongly immunogenic , and are thus of greatest importance for the experimental use of these animals , such as in transplantation and blood transfusion .
	manualset3
141712	4	408775	5	NULL	NULL	0	NULL	experimental use	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The antigens of the Drh system appear to be the most strongly immunogenic , and are thus of greatest importance for the experimental use of these animals , such as in transplantation and blood transfusion .
	manualset3
141713	5	408775	5	NULL	NULL	0	NULL	animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The antigens of the Drh system appear to be the most strongly immunogenic , and are thus of greatest importance for the experimental use of these animals , such as in transplantation and blood transfusion .
	manualset3
141714	6	408775	5	NULL	NULL	0	NULL	transplantation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The antigens of the Drh system appear to be the most strongly immunogenic , and are thus of greatest importance for the experimental use of these animals , such as in transplantation and blood transfusion .
	manualset3
141715	7	408775	5	NULL	NULL	0	NULL	blood transfusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The antigens of the Drh system appear to be the most strongly immunogenic , and are thus of greatest importance for the experimental use of these animals , such as in transplantation and blood transfusion .
	manualset3
141716	1	408776	5	NULL	NULL	0	NULL	antihypertensive actions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The antihypertensive actions of angiotensin - ( 1-7 ) are mediated by an angiotensin receptor that is distinct from the pharmacologically characterized AT1 or AT2 receptor subtypes .
	manualset3
141717	2	408776	5	NULL	NULL	0	NULL	angiotensin - ( 1-7 )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The antihypertensive actions of angiotensin - ( 1-7 ) are mediated by an angiotensin receptor that is distinct from the pharmacologically characterized AT1 or AT2 receptor subtypes .
	manualset3
141718	3	408776	5	NULL	NULL	0	NULL	angiotensin receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The antihypertensive actions of angiotensin - ( 1-7 ) are mediated by an angiotensin receptor that is distinct from the pharmacologically characterized AT1 or AT2 receptor subtypes .
	manualset3
141719	4	408776	5	NULL	NULL	NULL	NULL	AT1 receptor subtype	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The antihypertensive actions of angiotensin - ( 1-7 ) are mediated by an angiotensin receptor that is distinct from the pharmacologically characterized AT1 or AT2 receptor subtypes .
	manualset3
141720	5	408776	5	NULL	NULL	0	NULL	AT2 receptor subtype	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The antihypertensive actions of angiotensin - ( 1-7 ) are mediated by an angiotensin receptor that is distinct from the pharmacologically characterized AT1 or AT2 receptor subtypes .
	manualset3
141721	1	408777	5	NULL	NULL	0	NULL	antimalaria activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The antimalaria activity mediated by alpha-GalCer is stage-specific , since the course of blood-stage-induced infection was not inhibited by administration of this glycolipid .
	manualset3
141722	2	408777	5	NULL	NULL	NULL	NULL	alpha-GalCer	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The antimalaria activity mediated by alpha-GalCer is stage-specific , since the course of blood-stage-induced infection was not inhibited by administration of this glycolipid .
	manualset3
141723	3	408777	5	NULL	NULL	0	NULL	course of blood-stage-induced infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The antimalaria activity mediated by alpha-GalCer is stage-specific , since the course of blood-stage-induced infection was not inhibited by administration of this glycolipid .
	manualset3
141724	4	408777	5	NULL	NULL	0	NULL	administration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The antimalaria activity mediated by alpha-GalCer is stage-specific , since the course of blood-stage-induced infection was not inhibited by administration of this glycolipid .
	manualset3
141725	5	408777	5	NULL	NULL	0	NULL	glycolipid 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The antimalaria activity mediated by alpha-GalCer is stage-specific , since the course of blood-stage-induced infection was not inhibited by administration of this glycolipid .
	manualset3
141726	1	408778	5	NULL	NULL	0	NULL	antimicrobial activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The antimicrobial activity of copper and copper alloys against nosocomial pathogens and Mycobacterium tuberculosis isolated from healthcare facilities in the Western Cape : an in-vitro study .
	manualset3
141727	2	408778	5	NULL	NULL	0	NULL	copper 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The antimicrobial activity of copper and copper alloys against nosocomial pathogens and Mycobacterium tuberculosis isolated from healthcare facilities in the Western Cape : an in-vitro study .
	manualset3
141728	3	408778	5	NULL	NULL	0	NULL	copper alloys	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The antimicrobial activity of copper and copper alloys against nosocomial pathogens and Mycobacterium tuberculosis isolated from healthcare facilities in the Western Cape : an in-vitro study .
	manualset3
141729	4	408778	5	NULL	NULL	0	NULL	nosocomial pathogens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The antimicrobial activity of copper and copper alloys against nosocomial pathogens and Mycobacterium tuberculosis isolated from healthcare facilities in the Western Cape : an in-vitro study .
	manualset3
141730	5	408778	5	NULL	NULL	0	NULL	Mycobacterium tuberculosis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The antimicrobial activity of copper and copper alloys against nosocomial pathogens and Mycobacterium tuberculosis isolated from healthcare facilities in the Western Cape : an in-vitro study .
	manualset3
141731	6	408778	5	NULL	NULL	0	NULL	healthcare facilities	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The antimicrobial activity of copper and copper alloys against nosocomial pathogens and Mycobacterium tuberculosis isolated from healthcare facilities in the Western Cape : an in-vitro study .
	manualset3
141732	7	408778	5	NULL	NULL	0	NULL	Western Cape	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The antimicrobial activity of copper and copper alloys against nosocomial pathogens and Mycobacterium tuberculosis isolated from healthcare facilities in the Western Cape : an in-vitro study .
	manualset3
141733	8	408778	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The antimicrobial activity of copper and copper alloys against nosocomial pathogens and Mycobacterium tuberculosis isolated from healthcare facilities in the Western Cape : an in-vitro study .
	manualset3
141734	1	408779	5	NULL	NULL	0	NULL	antiobesity effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The antiobesity effect of wild ginseng ( WG ; Panax ginseng C.A. Meyer ) in male obese leptin-deficient ( B6.V-Lepob , ` ob/ob ' ) mice was evaluated .
	manualset3
141735	2	408779	5	NULL	NULL	0	NULL	wild ginseng ( WG ; Panax ginseng C.A. Meyer )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The antiobesity effect of wild ginseng ( WG ; Panax ginseng C.A. Meyer ) in male obese leptin-deficient ( B6.V-Lepob , ` ob/ob ' ) mice was evaluated .
	manualset3
141736	3	408779	5	NULL	NULL	0	NULL	male obese leptin-deficient ( B6.V-Lepob , ` ob/ob ' ) mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The antiobesity effect of wild ginseng ( WG ; Panax ginseng C.A. Meyer ) in male obese leptin-deficient ( B6.V-Lepob , ` ob/ob ' ) mice was evaluated .
	manualset3
141737	1	408780	5	NULL	NULL	0	NULL	antioxidant activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The antioxidant activity of all hexane extracts was evaluated by the 2 , 2-diphenyl-1-picrylhydrazyl ( DPPH ) radical scavenging method .
	manualset3
141738	2	408780	5	NULL	NULL	0	NULL	hexane extracts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The antioxidant activity of all hexane extracts was evaluated by the 2 , 2-diphenyl-1-picrylhydrazyl ( DPPH ) radical scavenging method .
	manualset3
141739	3	408780	5	NULL	NULL	0	NULL	2 , 2-diphenyl-1-picrylhydrazyl ( DPPH ) radical scavenging method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The antioxidant activity of all hexane extracts was evaluated by the 2 , 2-diphenyl-1-picrylhydrazyl ( DPPH ) radical scavenging method .
	manualset3
141740	1	408781	5	NULL	NULL	0	NULL	antioxidant , MnTnHex-2-PyP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The antioxidants , MnTnHex-2-PyP and Ascorbate and Trolox combination , significantly decreased postnatal motor deficits and extent of RepReOx .
	manualset3
141741	2	408781	5	NULL	NULL	0	NULL	antioxidant Ascorbate and Trolox combination 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The antioxidants , MnTnHex-2-PyP and Ascorbate and Trolox combination , significantly decreased postnatal motor deficits and extent of RepReOx .
	manualset3
141742	3	408781	5	NULL	NULL	0	NULL	postnatal motor deficits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The antioxidants , MnTnHex-2-PyP and Ascorbate and Trolox combination , significantly decreased postnatal motor deficits and extent of RepReOx .
	manualset3
141743	4	408781	5	NULL	NULL	0	NULL	RepReOx 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The antioxidants , MnTnHex-2-PyP and Ascorbate and Trolox combination , significantly decreased postnatal motor deficits and extent of RepReOx .
	manualset3
141744	1	408782	5	NULL	NULL	0	NULL	antioxidative properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The antioxidative properties of vanillic acid esters were systematically evaluated by multiple assays to compare with the well-known antioxidants , vanillic acid and Trolox .
	manualset3
141745	2	408782	5	NULL	NULL	0	NULL	vanillic acid esters	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The antioxidative properties of vanillic acid esters were systematically evaluated by multiple assays to compare with the well-known antioxidants , vanillic acid and Trolox .
	manualset3
141746	3	408782	5	NULL	NULL	0	NULL	multiple assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The antioxidative properties of vanillic acid esters were systematically evaluated by multiple assays to compare with the well-known antioxidants , vanillic acid and Trolox .
	manualset3
141747	4	408782	5	NULL	NULL	0	NULL	 antioxidant vanillic acid	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The antioxidative properties of vanillic acid esters were systematically evaluated by multiple assays to compare with the well-known antioxidants , vanillic acid and Trolox .
	manualset3
141748	5	408782	5	NULL	NULL	0	NULL	antioxidant Trolox 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The antioxidative properties of vanillic acid esters were systematically evaluated by multiple assays to compare with the well-known antioxidants , vanillic acid and Trolox .
	manualset3
141749	1	408783	5	NULL	NULL	0	NULL	antitumor protection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The antitumor protection was very weak in young Mice : no effect on mortality rate , only an increase in mean survival time was observed .
	manualset3
141750	2	408783	5	NULL	NULL	0	NULL	young Mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The antitumor protection was very weak in young Mice : no effect on mortality rate , only an increase in mean survival time was observed .
	manualset3
141751	3	408783	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The antitumor protection was very weak in young Mice : no effect on mortality rate , only an increase in mean survival time was observed .
	manualset3
141752	4	408783	5	NULL	NULL	0	NULL	mortality rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The antitumor protection was very weak in young Mice : no effect on mortality rate , only an increase in mean survival time was observed .
	manualset3
141753	5	408783	5	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The antitumor protection was very weak in young Mice : no effect on mortality rate , only an increase in mean survival time was observed .
	manualset3
141754	6	408783	5	NULL	NULL	0	NULL	mean survival time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The antitumor protection was very weak in young Mice : no effect on mortality rate , only an increase in mean survival time was observed .
	manualset3
141755	1	408784	5	NULL	NULL	0	NULL	antiviral activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The antiviral activity of the phenanthrene derivatives 1-6 , of the spyrostane triglycosides dioscin ( 7 ) and gracillin ( 8 ) , of the furostanol tetraglycosides methylprotodioscin ( 9 ) , its ( 25S ) epimer methylprotoneodioscin ( 10 ) , and methylprotogracillin 11 , have been tested towards two RNA viruses : vesicular stomatitis virus and human rhinovirus type 1B .
	manualset3
141756	2	408784	5	NULL	NULL	NULL	NULL	phenanthrene derivatives 1-6 , of the spyrostane triglycoside dioscin	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The antiviral activity of the phenanthrene derivatives 1-6 , of the spyrostane triglycosides dioscin ( 7 ) and gracillin ( 8 ) , of the furostanol tetraglycosides methylprotodioscin ( 9 ) , its ( 25S ) epimer methylprotoneodioscin ( 10 ) , and methylprotogracillin 11 , have been tested towards two RNA viruses : vesicular stomatitis virus and human rhinovirus type 1B .
	manualset3
141757	3	408784	5	NULL	NULL	0	NULL	phenanthrene derivatives 1-6 , of the spyrostane triglycoside gracillin	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The antiviral activity of the phenanthrene derivatives 1-6 , of the spyrostane triglycosides dioscin ( 7 ) and gracillin ( 8 ) , of the furostanol tetraglycosides methylprotodioscin ( 9 ) , its ( 25S ) epimer methylprotoneodioscin ( 10 ) , and methylprotogracillin 11 , have been tested towards two RNA viruses : vesicular stomatitis virus and human rhinovirus type 1B .
	manualset3
141758	4	408784	5	NULL	NULL	0	NULL	phenanthrene derivatives 1-6 , of the furostanol tetraglycosides methylprotodioscin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The antiviral activity of the phenanthrene derivatives 1-6 , of the spyrostane triglycosides dioscin ( 7 ) and gracillin ( 8 ) , of the furostanol tetraglycosides methylprotodioscin ( 9 ) , its ( 25S ) epimer methylprotoneodioscin ( 10 ) , and methylprotogracillin 11 , have been tested towards two RNA viruses : vesicular stomatitis virus and human rhinovirus type 1B .
	manualset3
141759	5	408784	5	NULL	NULL	0	NULL	( 25S ) epimer methylprotoneodioscin	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The antiviral activity of the phenanthrene derivatives 1-6 , of the spyrostane triglycosides dioscin ( 7 ) and gracillin ( 8 ) , of the furostanol tetraglycosides methylprotodioscin ( 9 ) , its ( 25S ) epimer methylprotoneodioscin ( 10 ) , and methylprotogracillin 11 , have been tested towards two RNA viruses : vesicular stomatitis virus and human rhinovirus type 1B .
	manualset3
141760	6	408784	5	NULL	NULL	0	NULL	methylprotogracillin 11	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The antiviral activity of the phenanthrene derivatives 1-6 , of the spyrostane triglycosides dioscin ( 7 ) and gracillin ( 8 ) , of the furostanol tetraglycosides methylprotodioscin ( 9 ) , its ( 25S ) epimer methylprotoneodioscin ( 10 ) , and methylprotogracillin 11 , have been tested towards two RNA viruses : vesicular stomatitis virus and human rhinovirus type 1B .
	manualset3
141761	7	408784	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The antiviral activity of the phenanthrene derivatives 1-6 , of the spyrostane triglycosides dioscin ( 7 ) and gracillin ( 8 ) , of the furostanol tetraglycosides methylprotodioscin ( 9 ) , its ( 25S ) epimer methylprotoneodioscin ( 10 ) , and methylprotogracillin 11 , have been tested towards two RNA viruses : vesicular stomatitis virus and human rhinovirus type 1B .
	manualset3
141762	8	408784	5	NULL	NULL	0	NULL	RNA viruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The antiviral activity of the phenanthrene derivatives 1-6 , of the spyrostane triglycosides dioscin ( 7 ) and gracillin ( 8 ) , of the furostanol tetraglycosides methylprotodioscin ( 9 ) , its ( 25S ) epimer methylprotoneodioscin ( 10 ) , and methylprotogracillin 11 , have been tested towards two RNA viruses : vesicular stomatitis virus and human rhinovirus type 1B .
	manualset3
141763	9	408784	5	NULL	NULL	0	NULL	vesicular stomatitis virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The antiviral activity of the phenanthrene derivatives 1-6 , of the spyrostane triglycosides dioscin ( 7 ) and gracillin ( 8 ) , of the furostanol tetraglycosides methylprotodioscin ( 9 ) , its ( 25S ) epimer methylprotoneodioscin ( 10 ) , and methylprotogracillin 11 , have been tested towards two RNA viruses : vesicular stomatitis virus and human rhinovirus type 1B .
	manualset3
141764	10	408784	5	NULL	NULL	0	NULL	human rhinovirus type 1B	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The antiviral activity of the phenanthrene derivatives 1-6 , of the spyrostane triglycosides dioscin ( 7 ) and gracillin ( 8 ) , of the furostanol tetraglycosides methylprotodioscin ( 9 ) , its ( 25S ) epimer methylprotoneodioscin ( 10 ) , and methylprotogracillin 11 , have been tested towards two RNA viruses : vesicular stomatitis virus and human rhinovirus type 1B .
	manualset3
141765	1	408785	5	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A role for the juxtamembrane domain of beta-dystroglycan in agrin-induced acetylcholine receptor clustering .
	manualset3
141766	2	408785	5	NULL	NULL	NULL	NULL	juxtamembrane domain of beta-dystroglycan	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A role for the juxtamembrane domain of beta-dystroglycan in agrin-induced acetylcholine receptor clustering .
	manualset3
141767	3	408785	5	NULL	NULL	0	NULL	agrin-induced acetylcholine receptor clustering	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A role for the juxtamembrane domain of beta-dystroglycan in agrin-induced acetylcholine receptor clustering .
	manualset3
141768	1	408786	5	NULL	NULL	0	NULL	apical-to-basolateral transcellular transport	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The apical-to-basolateral transcellular transport of genistein across a Caco-2 cell monolayer was significantly greater than that in the opposite direction .
	manualset3
141769	2	408786	5	NULL	NULL	0	NULL	genistein 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The apical-to-basolateral transcellular transport of genistein across a Caco-2 cell monolayer was significantly greater than that in the opposite direction .
	manualset3
141770	3	408786	5	NULL	NULL	0	NULL	Caco-2 cell monolayer	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The apical-to-basolateral transcellular transport of genistein across a Caco-2 cell monolayer was significantly greater than that in the opposite direction .
	manualset3
141771	4	408786	5	NULL	NULL	0	NULL	opposite direction 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The apical-to-basolateral transcellular transport of genistein across a Caco-2 cell monolayer was significantly greater than that in the opposite direction .
	manualset3
141772	1	408787	5	NULL	NULL	0	NULL	apparent molecular weight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The apparent molecular weight of both beta-N-acetylhexosaminidase A and B is about 100 , 000 when estimated with gel filtration column chromatography and the pH optimum for both is 4.0 .
	manualset3
141773	2	408787	5	NULL	NULL	0	NULL	beta-N-acetylhexosaminidase A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The apparent molecular weight of both beta-N-acetylhexosaminidase A and B is about 100 , 000 when estimated with gel filtration column chromatography and the pH optimum for both is 4.0 .
	manualset3
141774	3	408787	5	NULL	NULL	0	NULL	beta-N-acetylhexosaminidase B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The apparent molecular weight of both beta-N-acetylhexosaminidase A and B is about 100 , 000 when estimated with gel filtration column chromatography and the pH optimum for both is 4.0 .
	manualset3
141775	4	408787	5	NULL	NULL	0	NULL	100 , 000	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The apparent molecular weight of both beta-N-acetylhexosaminidase A and B is about 100 , 000 when estimated with gel filtration column chromatography and the pH optimum for both is 4.0 .
	manualset3
141776	5	408787	5	NULL	NULL	0	NULL	gel filtration column chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The apparent molecular weight of both beta-N-acetylhexosaminidase A and B is about 100 , 000 when estimated with gel filtration column chromatography and the pH optimum for both is 4.0 .
	manualset3
141777	6	408787	5	NULL	NULL	0	NULL	pH optimum	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The apparent molecular weight of both beta-N-acetylhexosaminidase A and B is about 100 , 000 when estimated with gel filtration column chromatography and the pH optimum for both is 4.0 .
	manualset3
141778	7	408787	5	NULL	NULL	0	NULL	4.0 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The apparent molecular weight of both beta-N-acetylhexosaminidase A and B is about 100 , 000 when estimated with gel filtration column chromatography and the pH optimum for both is 4.0 .
	manualset3
141779	1	408788	5	NULL	NULL	0	NULL	apparent rate constants ( k ( app ) ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The apparent rate constants ( k ( app ) ) were higher for UV/NO ( 3 ) ( - ) systems than for UV/HNO ( 2 ) / NO ( 2 ) ( - ) systems at high additive concentrations , whereas the opposite trend was observed for low additive concentrations .
	manualset3
141780	2	408788	5	NULL	NULL	0	NULL	UV/NO ( 3 ) ( - ) systems	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The apparent rate constants ( k ( app ) ) were higher for UV/NO ( 3 ) ( - ) systems than for UV/HNO ( 2 ) / NO ( 2 ) ( - ) systems at high additive concentrations , whereas the opposite trend was observed for low additive concentrations .
	manualset3
141781	3	408788	5	NULL	NULL	0	NULL	UV/HNO ( 2 ) / NO ( 2 ) ( - ) systems	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The apparent rate constants ( k ( app ) ) were higher for UV/NO ( 3 ) ( - ) systems than for UV/HNO ( 2 ) / NO ( 2 ) ( - ) systems at high additive concentrations , whereas the opposite trend was observed for low additive concentrations .
	manualset3
141782	4	408788	5	NULL	NULL	0	NULL	high additive concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The apparent rate constants ( k ( app ) ) were higher for UV/NO ( 3 ) ( - ) systems than for UV/HNO ( 2 ) / NO ( 2 ) ( - ) systems at high additive concentrations , whereas the opposite trend was observed for low additive concentrations .
	manualset3
141783	5	408788	5	NULL	NULL	0	NULL	opposite trend 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The apparent rate constants ( k ( app ) ) were higher for UV/NO ( 3 ) ( - ) systems than for UV/HNO ( 2 ) / NO ( 2 ) ( - ) systems at high additive concentrations , whereas the opposite trend was observed for low additive concentrations .
	manualset3
141784	6	408788	5	NULL	NULL	0	NULL	low additive concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The apparent rate constants ( k ( app ) ) were higher for UV/NO ( 3 ) ( - ) systems than for UV/HNO ( 2 ) / NO ( 2 ) ( - ) systems at high additive concentrations , whereas the opposite trend was observed for low additive concentrations .
	manualset3
141785	1	408789	5	NULL	NULL	0	NULL	apparent sedimentation coefficient	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The apparent sedimentation coefficient of the polymerase activity in the absence of salt is 8.4 S ( Mr = 180000-200000 ) , that in its presence ( 0.6 M NaCl or 0.12 M KCl ) being 6.3 S ( Mr = 80000-100000 ) .
	manualset3
141786	2	408789	5	NULL	NULL	0	NULL	polymerase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The apparent sedimentation coefficient of the polymerase activity in the absence of salt is 8.4 S ( Mr = 180000-200000 ) , that in its presence ( 0.6 M NaCl or 0.12 M KCl ) being 6.3 S ( Mr = 80000-100000 ) .
	manualset3
141787	3	408789	5	NULL	NULL	0	NULL	absence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The apparent sedimentation coefficient of the polymerase activity in the absence of salt is 8.4 S ( Mr = 180000-200000 ) , that in its presence ( 0.6 M NaCl or 0.12 M KCl ) being 6.3 S ( Mr = 80000-100000 ) .
	manualset3
141788	4	408789	5	NULL	NULL	0	NULL	salt 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The apparent sedimentation coefficient of the polymerase activity in the absence of salt is 8.4 S ( Mr = 180000-200000 ) , that in its presence ( 0.6 M NaCl or 0.12 M KCl ) being 6.3 S ( Mr = 80000-100000 ) .
	manualset3
141789	5	408789	5	NULL	NULL	0	NULL	8.4 S ( Mr = 180000-200000 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The apparent sedimentation coefficient of the polymerase activity in the absence of salt is 8.4 S ( Mr = 180000-200000 ) , that in its presence ( 0.6 M NaCl or 0.12 M KCl ) being 6.3 S ( Mr = 80000-100000 ) .
	manualset3
141790	6	408789	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The apparent sedimentation coefficient of the polymerase activity in the absence of salt is 8.4 S ( Mr = 180000-200000 ) , that in its presence ( 0.6 M NaCl or 0.12 M KCl ) being 6.3 S ( Mr = 80000-100000 ) .
	manualset3
141791	7	408789	5	NULL	NULL	0	NULL	 0.6 M NaCl 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The apparent sedimentation coefficient of the polymerase activity in the absence of salt is 8.4 S ( Mr = 180000-200000 ) , that in its presence ( 0.6 M NaCl or 0.12 M KCl ) being 6.3 S ( Mr = 80000-100000 ) .
	manualset3
141792	8	408789	5	NULL	NULL	0	NULL	0.12 M KCl	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The apparent sedimentation coefficient of the polymerase activity in the absence of salt is 8.4 S ( Mr = 180000-200000 ) , that in its presence ( 0.6 M NaCl or 0.12 M KCl ) being 6.3 S ( Mr = 80000-100000 ) .
	manualset3
141793	9	408789	5	NULL	NULL	0	NULL	6.3 S ( Mr = 80000-100000 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The apparent sedimentation coefficient of the polymerase activity in the absence of salt is 8.4 S ( Mr = 180000-200000 ) , that in its presence ( 0.6 M NaCl or 0.12 M KCl ) being 6.3 S ( Mr = 80000-100000 ) .
	manualset3
141794	1	408790	5	NULL	NULL	0	NULL	applicability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The applicability of the device has been finally demonstrated by the detection of rabbit IgG as model protein after an immunoassay performed on magnetic particles as immobilization platform .
	manualset3
141795	2	408790	5	NULL	NULL	0	NULL	device 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The applicability of the device has been finally demonstrated by the detection of rabbit IgG as model protein after an immunoassay performed on magnetic particles as immobilization platform .
	manualset3
141796	3	408790	5	NULL	NULL	0	NULL	detection 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The applicability of the device has been finally demonstrated by the detection of rabbit IgG as model protein after an immunoassay performed on magnetic particles as immobilization platform .
	manualset3
141797	4	408790	5	NULL	NULL	0	NULL	rabbit IgG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The applicability of the device has been finally demonstrated by the detection of rabbit IgG as model protein after an immunoassay performed on magnetic particles as immobilization platform .
	manualset3
141798	5	408790	5	NULL	NULL	0	NULL	model protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The applicability of the device has been finally demonstrated by the detection of rabbit IgG as model protein after an immunoassay performed on magnetic particles as immobilization platform .
	manualset3
141799	6	408790	5	NULL	NULL	0	NULL	immunoassay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The applicability of the device has been finally demonstrated by the detection of rabbit IgG as model protein after an immunoassay performed on magnetic particles as immobilization platform .
	manualset3
141800	7	408790	5	NULL	NULL	0	NULL	magnetic particles	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The applicability of the device has been finally demonstrated by the detection of rabbit IgG as model protein after an immunoassay performed on magnetic particles as immobilization platform .
	manualset3
141801	8	408790	5	NULL	NULL	0	NULL	immobilization platform	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The applicability of the device has been finally demonstrated by the detection of rabbit IgG as model protein after an immunoassay performed on magnetic particles as immobilization platform .
	manualset3
141802	1	408791	5	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of Fortify ( Bisco , Lombard , IL ) , an unfilled resin , to the surface of composite resin restorations is intended to fill in defects in the surface that persist despite polishing , improve marginal integrity , and increase these materials ' resistance to abrasion .
	manualset3
141803	2	408791	5	NULL	NULL	0	NULL	Fortify ( Bisco , Lombard , IL ) , an unfilled resin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of Fortify ( Bisco , Lombard , IL ) , an unfilled resin , to the surface of composite resin restorations is intended to fill in defects in the surface that persist despite polishing , improve marginal integrity , and increase these materials ' resistance to abrasion .
	manualset3
141804	3	408791	5	NULL	NULL	0	NULL	surface	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of Fortify ( Bisco , Lombard , IL ) , an unfilled resin , to the surface of composite resin restorations is intended to fill in defects in the surface that persist despite polishing , improve marginal integrity , and increase these materials ' resistance to abrasion .
	manualset3
141805	4	408791	5	NULL	NULL	0	NULL	composite resin restorations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of Fortify ( Bisco , Lombard , IL ) , an unfilled resin , to the surface of composite resin restorations is intended to fill in defects in the surface that persist despite polishing , improve marginal integrity , and increase these materials ' resistance to abrasion .
	manualset3
141806	5	408791	5	NULL	NULL	0	NULL	defects	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of Fortify ( Bisco , Lombard , IL ) , an unfilled resin , to the surface of composite resin restorations is intended to fill in defects in the surface that persist despite polishing , improve marginal integrity , and increase these materials ' resistance to abrasion .
	manualset3
141807	6	408791	5	NULL	NULL	0	NULL	surface	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of Fortify ( Bisco , Lombard , IL ) , an unfilled resin , to the surface of composite resin restorations is intended to fill in defects in the surface that persist despite polishing , improve marginal integrity , and increase these materials ' resistance to abrasion .
	manualset3
141808	7	408791	5	NULL	NULL	0	NULL	marginal integrity	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of Fortify ( Bisco , Lombard , IL ) , an unfilled resin , to the surface of composite resin restorations is intended to fill in defects in the surface that persist despite polishing , improve marginal integrity , and increase these materials ' resistance to abrasion .
	manualset3
141809	8	408791	5	NULL	NULL	0	NULL	resistance to abrasion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of Fortify ( Bisco , Lombard , IL ) , an unfilled resin , to the surface of composite resin restorations is intended to fill in defects in the surface that persist despite polishing , improve marginal integrity , and increase these materials ' resistance to abrasion .
	manualset3
141810	1	408792	5	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of a silage inoculant led to increased enterococci counts , but not streptococci counts , in corn samples following the ensiling period .
	manualset3
141811	2	408792	5	NULL	NULL	0	NULL	silage inoculant	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of a silage inoculant led to increased enterococci counts , but not streptococci counts , in corn samples following the ensiling period .
	manualset3
141812	3	408792	5	NULL	NULL	0	NULL	 enterococci counts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of a silage inoculant led to increased enterococci counts , but not streptococci counts , in corn samples following the ensiling period .
	manualset3
141813	4	408792	5	NULL	NULL	0	NULL	 streptococci counts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of a silage inoculant led to increased enterococci counts , but not streptococci counts , in corn samples following the ensiling period .
	manualset3
141814	5	408792	5	NULL	NULL	0	NULL	corn samples	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of a silage inoculant led to increased enterococci counts , but not streptococci counts , in corn samples following the ensiling period .
	manualset3
141815	6	408792	5	NULL	NULL	0	NULL	ensiling period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of a silage inoculant led to increased enterococci counts , but not streptococci counts , in corn samples following the ensiling period .
	manualset3
141816	1	408793	5	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of hormone examinations , color Doppler and Rigiscan exams help at establishing diagnoses .
	manualset3
141817	2	408793	5	NULL	NULL	NULL	NULL	hormone examinations	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The application of hormone examinations , color Doppler and Rigiscan exams help at establishing diagnoses .
	manualset3
141818	3	408793	5	NULL	NULL	0	NULL	color Doppler exams	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of hormone examinations , color Doppler and Rigiscan exams help at establishing diagnoses .
	manualset3
141819	4	408793	5	NULL	NULL	0	NULL	Rigiscan exams	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of hormone examinations , color Doppler and Rigiscan exams help at establishing diagnoses .
	manualset3
141820	5	408793	5	NULL	NULL	0	NULL	diagnoses	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of hormone examinations , color Doppler and Rigiscan exams help at establishing diagnoses .
	manualset3
141821	1	408794	5	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A role of exogenous female hormones ( i.e. oral contraceptives and hormone replacement therapy ( HRT ) in such different trends is possible .
	manualset3
141822	2	408794	5	NULL	NULL	0	NULL	exogenous female hormones	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A role of exogenous female hormones ( i.e. oral contraceptives and hormone replacement therapy ( HRT ) in such different trends is possible .
	manualset3
141823	3	408794	5	NULL	NULL	0	NULL	oral contraceptives	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A role of exogenous female hormones ( i.e. oral contraceptives and hormone replacement therapy ( HRT ) in such different trends is possible .
	manualset3
141824	4	408794	5	NULL	NULL	0	NULL	hormone replacement therapy ( HRT )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A role of exogenous female hormones ( i.e. oral contraceptives and hormone replacement therapy ( HRT ) in such different trends is possible .
	manualset3
141825	5	408794	5	NULL	NULL	0	NULL	trends	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A role of exogenous female hormones ( i.e. oral contraceptives and hormone replacement therapy ( HRT ) in such different trends is possible .
	manualset3
141826	1	408795	5	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of thermal treatment in medicine has truly developed during the last decade .
	manualset3
141827	2	408795	5	NULL	NULL	0	NULL	thermal treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of thermal treatment in medicine has truly developed during the last decade .
	manualset3
141828	3	408795	5	NULL	NULL	0	NULL	medicine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of thermal treatment in medicine has truly developed during the last decade .
	manualset3
141829	4	408795	5	NULL	NULL	0	NULL	last decade	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of thermal treatment in medicine has truly developed during the last decade .
	manualset3
141830	1	408796	5	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of xeroradiography to nearly every aspect of diagnostic radiology has been attempted .
	manualset3
141831	2	408796	5	NULL	NULL	0	NULL	xeroradiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of xeroradiography to nearly every aspect of diagnostic radiology has been attempted .
	manualset3
141832	3	408796	5	NULL	NULL	0	NULL	aspect	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of xeroradiography to nearly every aspect of diagnostic radiology has been attempted .
	manualset3
141833	4	408796	5	NULL	NULL	0	NULL	diagnostic radiology	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of xeroradiography to nearly every aspect of diagnostic radiology has been attempted .
	manualset3
141834	1	408797	5	NULL	NULL	0	NULL	appreciation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The appreciation of the importance of cell biology in explaining why cells become resistant to anticancer drugs has developed rapidly , and examples are given .
	manualset3
141835	2	408797	5	NULL	NULL	0	NULL	importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The appreciation of the importance of cell biology in explaining why cells become resistant to anticancer drugs has developed rapidly , and examples are given .
	manualset3
141836	3	408797	5	NULL	NULL	0	NULL	cell biology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The appreciation of the importance of cell biology in explaining why cells become resistant to anticancer drugs has developed rapidly , and examples are given .
	manualset3
141837	4	408797	5	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The appreciation of the importance of cell biology in explaining why cells become resistant to anticancer drugs has developed rapidly , and examples are given .
	manualset3
141838	5	408797	5	NULL	NULL	0	NULL	anticancer drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The appreciation of the importance of cell biology in explaining why cells become resistant to anticancer drugs has developed rapidly , and examples are given .
	manualset3
141839	6	408797	5	NULL	NULL	0	NULL	examples	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The appreciation of the importance of cell biology in explaining why cells become resistant to anticancer drugs has developed rapidly , and examples are given .
	manualset3
141840	1	408798	5	NULL	NULL	0	NULL	approach	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The approach can use any standard sequence-element-to-element probabilistic similarity measures and affine gap penalty functions .
	manualset3
141841	2	408798	5	NULL	NULL	0	NULL	standard sequence-element-to-element probabilistic similarity measures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The approach can use any standard sequence-element-to-element probabilistic similarity measures and affine gap penalty functions .
	manualset3
141842	3	408798	5	NULL	NULL	0	NULL	affine gap penalty functions	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The approach can use any standard sequence-element-to-element probabilistic similarity measures and affine gap penalty functions .
	manualset3
141843	1	408799	5	NULL	NULL	0	NULL	aqueous extract 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The aqueous extract of orthosiphon thymiflorus produced significant inhibitory effect on the dose response curve of acetyl choline .
	manualset3
141844	2	408799	5	NULL	NULL	0	NULL	orthosiphon thymiflorus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The aqueous extract of orthosiphon thymiflorus produced significant inhibitory effect on the dose response curve of acetyl choline .
	manualset3
141845	3	408799	5	NULL	NULL	0	NULL	significant inhibitory effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aqueous extract of orthosiphon thymiflorus produced significant inhibitory effect on the dose response curve of acetyl choline .
	manualset3
141846	4	408799	5	NULL	NULL	0	NULL	dose response curve	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The aqueous extract of orthosiphon thymiflorus produced significant inhibitory effect on the dose response curve of acetyl choline .
	manualset3
141847	5	408799	5	NULL	NULL	0	NULL	acetyl choline	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aqueous extract of orthosiphon thymiflorus produced significant inhibitory effect on the dose response curve of acetyl choline .
	manualset3
141848	1	408800	5	NULL	NULL	0	NULL	aqueous solutions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The aqueous solutions became yellow rapidly and progressively : the higher their pH , the more intense their coloration .
	manualset3
141849	2	408800	5	NULL	NULL	0	NULL	pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aqueous solutions became yellow rapidly and progressively : the higher their pH , the more intense their coloration .
	manualset3
141850	3	408800	5	NULL	NULL	0	NULL	coloration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aqueous solutions became yellow rapidly and progressively : the higher their pH , the more intense their coloration .
	manualset3
141851	1	408801	5	NULL	NULL	0	NULL	architecture	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The architecture utilizes modern advances in desktop microcomputers and has been designed so that vocal motor control laboratories ( or similar settings ) with modest funding can more fully participate in comprehensive investigations of speech production .
	manualset3
141852	2	408801	5	NULL	NULL	0	NULL	desktop microcomputers	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The architecture utilizes modern advances in desktop microcomputers and has been designed so that vocal motor control laboratories ( or similar settings ) with modest funding can more fully participate in comprehensive investigations of speech production .
	manualset3
141853	3	408801	5	NULL	NULL	0	NULL	vocal motor control laboratories	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The architecture utilizes modern advances in desktop microcomputers and has been designed so that vocal motor control laboratories ( or similar settings ) with modest funding can more fully participate in comprehensive investigations of speech production .
	manualset3
141854	4	408801	5	NULL	NULL	0	NULL	comprehensive investigations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The architecture utilizes modern advances in desktop microcomputers and has been designed so that vocal motor control laboratories ( or similar settings ) with modest funding can more fully participate in comprehensive investigations of speech production .
	manualset3
141855	5	408801	5	NULL	NULL	0	NULL	speech production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The architecture utilizes modern advances in desktop microcomputers and has been designed so that vocal motor control laboratories ( or similar settings ) with modest funding can more fully participate in comprehensive investigations of speech production .
	manualset3
144844	6	408801	5	NULL	NULL	0	NULL	modest funding	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The architecture utilizes modern advances in desktop microcomputers and has been designed so that vocal motor control laboratories ( or similar settings ) with modest funding can more fully participate in comprehensive investigations of speech production .
	manualset3
141856	1	408802	5	NULL	NULL	0	NULL	argument	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The argument of the stretched exponential decay p decreased monotonically as the temperature was lowered toward the gel point , until , at gelation , p approximately 0.5 .
	manualset3
141857	2	408802	5	NULL	NULL	0	NULL	stretched exponential decay p	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The argument of the stretched exponential decay p decreased monotonically as the temperature was lowered toward the gel point , until , at gelation , p approximately 0.5 .
	manualset3
141858	3	408802	5	NULL	NULL	0	NULL	temperature	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The argument of the stretched exponential decay p decreased monotonically as the temperature was lowered toward the gel point , until , at gelation , p approximately 0.5 .
	manualset3
141859	4	408802	5	NULL	NULL	0	NULL	gel point	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The argument of the stretched exponential decay p decreased monotonically as the temperature was lowered toward the gel point , until , at gelation , p approximately 0.5 .
	manualset3
141860	5	408802	5	NULL	NULL	0	NULL	gelation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The argument of the stretched exponential decay p decreased monotonically as the temperature was lowered toward the gel point , until , at gelation , p approximately 0.5 .
	manualset3
141861	6	408802	5	NULL	NULL	0	NULL	p	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The argument of the stretched exponential decay p decreased monotonically as the temperature was lowered toward the gel point , until , at gelation , p approximately 0.5 .
	manualset3
141862	7	408802	5	NULL	NULL	0	NULL	0.5	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The argument of the stretched exponential decay p decreased monotonically as the temperature was lowered toward the gel point , until , at gelation , p approximately 0.5 .
	manualset3
141863	1	408803	5	NULL	NULL	0	NULL	array	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The array of tropomyosin subunits present in a cell culture was reflected in the polypeptide chain pattern seen on SDS-polyacrylamide gels of microfilaments isolated from that culture .
	manualset3
141864	2	408803	5	NULL	NULL	0	NULL	tropomyosin subunits	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The array of tropomyosin subunits present in a cell culture was reflected in the polypeptide chain pattern seen on SDS-polyacrylamide gels of microfilaments isolated from that culture .
	manualset3
141865	3	408803	5	NULL	NULL	0	NULL	cell culture	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The array of tropomyosin subunits present in a cell culture was reflected in the polypeptide chain pattern seen on SDS-polyacrylamide gels of microfilaments isolated from that culture .
	manualset3
141866	4	408803	5	NULL	NULL	0	NULL	polypeptide chain pattern	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The array of tropomyosin subunits present in a cell culture was reflected in the polypeptide chain pattern seen on SDS-polyacrylamide gels of microfilaments isolated from that culture .
	manualset3
141867	5	408803	5	NULL	NULL	0	NULL	SDS-polyacrylamide gels	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The array of tropomyosin subunits present in a cell culture was reflected in the polypeptide chain pattern seen on SDS-polyacrylamide gels of microfilaments isolated from that culture .
	manualset3
141868	6	408803	5	NULL	NULL	0	NULL	microfilaments	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The array of tropomyosin subunits present in a cell culture was reflected in the polypeptide chain pattern seen on SDS-polyacrylamide gels of microfilaments isolated from that culture .
	manualset3
141869	7	408803	5	NULL	NULL	0	NULL	culture	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The array of tropomyosin subunits present in a cell culture was reflected in the polypeptide chain pattern seen on SDS-polyacrylamide gels of microfilaments isolated from that culture .
	manualset3
141870	1	408804	5	NULL	NULL	NULL	NULL	ars operon	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ars operon of the conjugative plasmid R773 encodes an anion pump .
	manualset3
141871	2	408804	5	NULL	NULL	0	NULL	conjugative plasmid R773	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The ars operon of the conjugative plasmid R773 encodes an anion pump .
	manualset3
141872	3	408804	5	NULL	NULL	0	NULL	anion pump	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The ars operon of the conjugative plasmid R773 encodes an anion pump .
	manualset3
141873	1	408805	5	NULL	NULL	0	NULL	arsB gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The arsB gene , which encodes a putative arsenite-specific efflux pump was highly induced by As3 + and As5 + ions , while other metal salts provoked insignificant transcript level increase .
	manualset3
141874	2	408805	5	NULL	NULL	0	NULL	putative arsenite-specific efflux pump	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The arsB gene , which encodes a putative arsenite-specific efflux pump was highly induced by As3 + and As5 + ions , while other metal salts provoked insignificant transcript level increase .
	manualset3
141875	3	408805	5	NULL	NULL	0	NULL	As3 + ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The arsB gene , which encodes a putative arsenite-specific efflux pump was highly induced by As3 + and As5 + ions , while other metal salts provoked insignificant transcript level increase .
	manualset3
141876	4	408805	5	NULL	NULL	0	NULL	As5 + ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The arsB gene , which encodes a putative arsenite-specific efflux pump was highly induced by As3 + and As5 + ions , while other metal salts provoked insignificant transcript level increase .
	manualset3
141877	5	408805	5	NULL	NULL	0	NULL	metal salts 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The arsB gene , which encodes a putative arsenite-specific efflux pump was highly induced by As3 + and As5 + ions , while other metal salts provoked insignificant transcript level increase .
	manualset3
141878	6	408805	5	NULL	NULL	0	NULL	transcript level increase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The arsB gene , which encodes a putative arsenite-specific efflux pump was highly induced by As3 + and As5 + ions , while other metal salts provoked insignificant transcript level increase .
	manualset3
141879	1	408806	5	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The article comments on the trainig of auxiliary personnel and the scope of their functions .
	manualset3
141880	3	408806	5	NULL	NULL	NULL	NULL	auxiliary personnel	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The article comments on the trainig of auxiliary personnel and the scope of their functions .
	manualset3
141881	2	408806	5	NULL	NULL	0	NULL	trainig	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The article comments on the trainig of auxiliary personnel and the scope of their functions .
	manualset3
141882	4	408806	5	NULL	NULL	0	NULL	scope	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The article comments on the trainig of auxiliary personnel and the scope of their functions .
	manualset3
141883	5	408806	5	NULL	NULL	0	NULL	functions	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The article comments on the trainig of auxiliary personnel and the scope of their functions .
	manualset3
141884	1	408807	5	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The article describes historical developments central to the emergence of the new terminology and describes the terminology , its attributes , and rules of application .
	manualset3
141885	2	408807	5	NULL	NULL	0	NULL	historical developments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The article describes historical developments central to the emergence of the new terminology and describes the terminology , its attributes , and rules of application .
	manualset3
141886	3	408807	5	NULL	NULL	0	NULL	emergence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The article describes historical developments central to the emergence of the new terminology and describes the terminology , its attributes , and rules of application .
	manualset3
141887	4	408807	5	NULL	NULL	0	NULL	terminology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The article describes historical developments central to the emergence of the new terminology and describes the terminology , its attributes , and rules of application .
	manualset3
141888	5	408807	5	NULL	NULL	0	NULL	terminology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The article describes historical developments central to the emergence of the new terminology and describes the terminology , its attributes , and rules of application .
	manualset3
141889	6	408807	5	NULL	NULL	0	NULL	rules of application	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The article describes historical developments central to the emergence of the new terminology and describes the terminology , its attributes , and rules of application .
	manualset3
141890	1	408808	5	NULL	NULL	0	NULL	articles	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The articles included in the study were identified using MEDLINE and Scopus databases and revised according to their title and abstract and , afterwards , their full text was read considering inclusion and exclusion criteria .
	manualset3
141891	2	408808	5	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The articles included in the study were identified using MEDLINE and Scopus databases and revised according to their title and abstract and , afterwards , their full text was read considering inclusion and exclusion criteria .
	manualset3
141892	3	408808	5	NULL	NULL	0	NULL	MEDLINE	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The articles included in the study were identified using MEDLINE and Scopus databases and revised according to their title and abstract and , afterwards , their full text was read considering inclusion and exclusion criteria .
	manualset3
141893	4	408808	5	NULL	NULL	0	NULL	Scopus databases	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The articles included in the study were identified using MEDLINE and Scopus databases and revised according to their title and abstract and , afterwards , their full text was read considering inclusion and exclusion criteria .
	manualset3
141894	5	408808	5	NULL	NULL	NULL	NULL	title	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The articles included in the study were identified using MEDLINE and Scopus databases and revised according to their title and abstract and , afterwards , their full text was read considering inclusion and exclusion criteria .
	manualset3
141895	6	408808	5	NULL	NULL	0	NULL	abstract	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The articles included in the study were identified using MEDLINE and Scopus databases and revised according to their title and abstract and , afterwards , their full text was read considering inclusion and exclusion criteria .
	manualset3
141896	7	408808	5	NULL	NULL	0	NULL	full text 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The articles included in the study were identified using MEDLINE and Scopus databases and revised according to their title and abstract and , afterwards , their full text was read considering inclusion and exclusion criteria .
	manualset3
141897	8	408808	5	NULL	NULL	0	NULL	inclusion criteria	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The articles included in the study were identified using MEDLINE and Scopus databases and revised according to their title and abstract and , afterwards , their full text was read considering inclusion and exclusion criteria .
	manualset3
141898	9	408808	5	NULL	NULL	0	NULL	exclusion criteria	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The articles included in the study were identified using MEDLINE and Scopus databases and revised according to their title and abstract and , afterwards , their full text was read considering inclusion and exclusion criteria .
	manualset3
141899	1	408809	5	NULL	NULL	0	NULL	aryl groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The aryl groups behave as bidirectional free rotors in three of the four isomers of the 360 rotation cycle , but rotation of the rotors is hindered in the fourth isomer .
	manualset3
141900	2	408809	5	NULL	NULL	NULL	NULL	bidirectional free rotors	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The aryl groups behave as bidirectional free rotors in three of the four isomers of the 360 rotation cycle , but rotation of the rotors is hindered in the fourth isomer .
	manualset3
141901	3	408809	5	NULL	NULL	0	NULL	three of the four	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The aryl groups behave as bidirectional free rotors in three of the four isomers of the 360 rotation cycle , but rotation of the rotors is hindered in the fourth isomer .
	manualset3
141902	4	408809	5	NULL	NULL	0	NULL	isomers	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aryl groups behave as bidirectional free rotors in three of the four isomers of the 360 rotation cycle , but rotation of the rotors is hindered in the fourth isomer .
	manualset3
141903	5	408809	5	NULL	NULL	0	NULL	360 rotation cycle	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The aryl groups behave as bidirectional free rotors in three of the four isomers of the 360 rotation cycle , but rotation of the rotors is hindered in the fourth isomer .
	manualset3
141904	6	408809	5	NULL	NULL	0	NULL	rotation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aryl groups behave as bidirectional free rotors in three of the four isomers of the 360 rotation cycle , but rotation of the rotors is hindered in the fourth isomer .
	manualset3
141905	7	408809	5	NULL	NULL	0	NULL	rotors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aryl groups behave as bidirectional free rotors in three of the four isomers of the 360 rotation cycle , but rotation of the rotors is hindered in the fourth isomer .
	manualset3
144845	8	408809	5	NULL	NULL	0	NULL	isomer 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aryl groups behave as bidirectional free rotors in three of the four isomers of the 360 rotation cycle , but rotation of the rotors is hindered in the fourth isomer .
	manualset3
141906	1	408810	5	NULL	NULL	0	NULL	fluorescent nanoparticles	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The as-prepared fluorescent nanoparticles showed rapid response , excellent stability and high reproducibility as pH sensors .
	manualset3
141907	2	408810	5	NULL	NULL	0	NULL	response	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The as-prepared fluorescent nanoparticles showed rapid response , excellent stability and high reproducibility as pH sensors .
	manualset3
141908	3	408810	5	NULL	NULL	0	NULL	excellent stability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The as-prepared fluorescent nanoparticles showed rapid response , excellent stability and high reproducibility as pH sensors .
	manualset3
141909	4	408810	5	NULL	NULL	0	NULL	high reproducibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The as-prepared fluorescent nanoparticles showed rapid response , excellent stability and high reproducibility as pH sensors .
	manualset3
141910	5	408810	5	NULL	NULL	0	NULL	 pH sensors	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The as-prepared fluorescent nanoparticles showed rapid response , excellent stability and high reproducibility as pH sensors .
	manualset3
141911	1	408811	5	NULL	NULL	0	NULL	aspiration cytodiagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aspiration cytodiagnosis was further confirmed by subsequent examination of cell blocks from the aspirated material and biopsy of the breast mass. .
	manualset3
141912	2	408811	5	NULL	NULL	0	NULL	subsequent examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aspiration cytodiagnosis was further confirmed by subsequent examination of cell blocks from the aspirated material and biopsy of the breast mass. .
	manualset3
141913	3	408811	5	NULL	NULL	0	NULL	cell blocks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aspiration cytodiagnosis was further confirmed by subsequent examination of cell blocks from the aspirated material and biopsy of the breast mass. .
	manualset3
141914	4	408811	5	NULL	NULL	0	NULL	aspirated material	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aspiration cytodiagnosis was further confirmed by subsequent examination of cell blocks from the aspirated material and biopsy of the breast mass. .
	manualset3
141915	5	408811	5	NULL	NULL	0	NULL	biopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aspiration cytodiagnosis was further confirmed by subsequent examination of cell blocks from the aspirated material and biopsy of the breast mass. .
	manualset3
141916	6	408811	5	NULL	NULL	NULL	NULL	breast mass	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The aspiration cytodiagnosis was further confirmed by subsequent examination of cell blocks from the aspirated material and biopsy of the breast mass. .
	manualset3
141917	1	408812	5	NULL	NULL	0	NULL	assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay also revealed chemical-induced accumulation of several binary multidrug transporter complexes that largely paralleled increases in transcript levels .
	manualset3
141918	2	408812	5	NULL	NULL	0	NULL	chemical-induced accumulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay also revealed chemical-induced accumulation of several binary multidrug transporter complexes that largely paralleled increases in transcript levels .
	manualset3
141919	3	408812	5	NULL	NULL	0	NULL	several binary multidrug transporter complexes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay also revealed chemical-induced accumulation of several binary multidrug transporter complexes that largely paralleled increases in transcript levels .
	manualset3
141920	4	408812	5	NULL	NULL	0	NULL	transcript levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay also revealed chemical-induced accumulation of several binary multidrug transporter complexes that largely paralleled increases in transcript levels .
	manualset3
141921	1	408813	5	NULL	NULL	0	NULL	assay detection range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay detection range spans five orders of magnitude , from 1 x 10 ( -3 ) to 1 x 10 ( -8 ) M. The assay element comprises of multilayer coated chip , containing the active reagents in an agarose matrix and a plastic module serving both as a holder and a spreader .
	manualset3
141922	2	408813	5	NULL	NULL	0	NULL	five orders of magnitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay detection range spans five orders of magnitude , from 1 x 10 ( -3 ) to 1 x 10 ( -8 ) M. The assay element comprises of multilayer coated chip , containing the active reagents in an agarose matrix and a plastic module serving both as a holder and a spreader .
	manualset3
141923	3	408813	5	NULL	NULL	0	NULL	1 x 10 ( -3 ) to 1 x 10 ( -8 ) M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay detection range spans five orders of magnitude , from 1 x 10 ( -3 ) to 1 x 10 ( -8 ) M. The assay element comprises of multilayer coated chip , containing the active reagents in an agarose matrix and a plastic module serving both as a holder and a spreader .
	manualset3
141924	4	408813	5	NULL	NULL	0	NULL	assay element	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay detection range spans five orders of magnitude , from 1 x 10 ( -3 ) to 1 x 10 ( -8 ) M. The assay element comprises of multilayer coated chip , containing the active reagents in an agarose matrix and a plastic module serving both as a holder and a spreader .
	manualset3
141925	5	408813	5	NULL	NULL	0	NULL	multilayer coated chip	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay detection range spans five orders of magnitude , from 1 x 10 ( -3 ) to 1 x 10 ( -8 ) M. The assay element comprises of multilayer coated chip , containing the active reagents in an agarose matrix and a plastic module serving both as a holder and a spreader .
	manualset3
141926	6	408813	5	NULL	NULL	0	NULL	active reagents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay detection range spans five orders of magnitude , from 1 x 10 ( -3 ) to 1 x 10 ( -8 ) M. The assay element comprises of multilayer coated chip , containing the active reagents in an agarose matrix and a plastic module serving both as a holder and a spreader .
	manualset3
141927	7	408813	5	NULL	NULL	0	NULL	agarose matrix	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay detection range spans five orders of magnitude , from 1 x 10 ( -3 ) to 1 x 10 ( -8 ) M. The assay element comprises of multilayer coated chip , containing the active reagents in an agarose matrix and a plastic module serving both as a holder and a spreader .
	manualset3
141928	8	408813	5	NULL	NULL	0	NULL	plastic module	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay detection range spans five orders of magnitude , from 1 x 10 ( -3 ) to 1 x 10 ( -8 ) M. The assay element comprises of multilayer coated chip , containing the active reagents in an agarose matrix and a plastic module serving both as a holder and a spreader .
	manualset3
141929	9	408813	5	NULL	NULL	0	NULL	holder	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay detection range spans five orders of magnitude , from 1 x 10 ( -3 ) to 1 x 10 ( -8 ) M. The assay element comprises of multilayer coated chip , containing the active reagents in an agarose matrix and a plastic module serving both as a holder and a spreader .
	manualset3
141930	10	408813	5	NULL	NULL	0	NULL	spreader	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay detection range spans five orders of magnitude , from 1 x 10 ( -3 ) to 1 x 10 ( -8 ) M. The assay element comprises of multilayer coated chip , containing the active reagents in an agarose matrix and a plastic module serving both as a holder and a spreader .
	manualset3
141931	1	408814	5	NULL	NULL	0	NULL	assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay for IL-6 mRNA was able to discriminate between samples with a two - to fourfold difference in concentration , had an intra-assay coefficient of variation ( CV ) of 17 % and an inter-assay CV of 24 % .
	manualset3
141932	2	408814	5	NULL	NULL	0	NULL	IL-6 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay for IL-6 mRNA was able to discriminate between samples with a two - to fourfold difference in concentration , had an intra-assay coefficient of variation ( CV ) of 17 % and an inter-assay CV of 24 % .
	manualset3
141933	3	408814	5	NULL	NULL	0	NULL	samples	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay for IL-6 mRNA was able to discriminate between samples with a two - to fourfold difference in concentration , had an intra-assay coefficient of variation ( CV ) of 17 % and an inter-assay CV of 24 % .
	manualset3
141934	4	408814	5	NULL	NULL	0	NULL	two - to fourfold difference	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay for IL-6 mRNA was able to discriminate between samples with a two - to fourfold difference in concentration , had an intra-assay coefficient of variation ( CV ) of 17 % and an inter-assay CV of 24 % .
	manualset3
141935	5	408814	5	NULL	NULL	0	NULL	concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay for IL-6 mRNA was able to discriminate between samples with a two - to fourfold difference in concentration , had an intra-assay coefficient of variation ( CV ) of 17 % and an inter-assay CV of 24 % .
	manualset3
141936	6	408814	5	NULL	NULL	0	NULL	intra-assay coefficient of variation ( CV )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay for IL-6 mRNA was able to discriminate between samples with a two - to fourfold difference in concentration , had an intra-assay coefficient of variation ( CV ) of 17 % and an inter-assay CV of 24 % .
	manualset3
141937	7	408814	5	NULL	NULL	0	NULL	17 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay for IL-6 mRNA was able to discriminate between samples with a two - to fourfold difference in concentration , had an intra-assay coefficient of variation ( CV ) of 17 % and an inter-assay CV of 24 % .
	manualset3
141938	8	408814	5	NULL	NULL	0	NULL	inter-assay CV	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay for IL-6 mRNA was able to discriminate between samples with a two - to fourfold difference in concentration , had an intra-assay coefficient of variation ( CV ) of 17 % and an inter-assay CV of 24 % .
	manualset3
141939	9	408814	5	NULL	NULL	0	NULL	24 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay for IL-6 mRNA was able to discriminate between samples with a two - to fourfold difference in concentration , had an intra-assay coefficient of variation ( CV ) of 17 % and an inter-assay CV of 24 % .
	manualset3
141940	1	408815	5	NULL	NULL	0	NULL	assay system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay system uses flex-vinyl microtiter plates on which bovine methyl albumin , the respective polynucleotide , a 1 : 80 dilution of patient serum , and tritiated high affinity anti-IgG , - IgA , or - IgM are layered .
	manualset3
141941	2	408815	5	NULL	NULL	0	NULL	flex-vinyl microtiter plates	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay system uses flex-vinyl microtiter plates on which bovine methyl albumin , the respective polynucleotide , a 1 : 80 dilution of patient serum , and tritiated high affinity anti-IgG , - IgA , or - IgM are layered .
	manualset3
141942	3	408815	5	NULL	NULL	0	NULL	bovine methyl albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay system uses flex-vinyl microtiter plates on which bovine methyl albumin , the respective polynucleotide , a 1 : 80 dilution of patient serum , and tritiated high affinity anti-IgG , - IgA , or - IgM are layered .
	manualset3
141943	4	408815	5	NULL	NULL	0	NULL	polynucleotide	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay system uses flex-vinyl microtiter plates on which bovine methyl albumin , the respective polynucleotide , a 1 : 80 dilution of patient serum , and tritiated high affinity anti-IgG , - IgA , or - IgM are layered .
	manualset3
141944	5	408815	5	NULL	NULL	0	NULL	1 : 80 dilution	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay system uses flex-vinyl microtiter plates on which bovine methyl albumin , the respective polynucleotide , a 1 : 80 dilution of patient serum , and tritiated high affinity anti-IgG , - IgA , or - IgM are layered .
	manualset3
141945	6	408815	5	NULL	NULL	0	NULL	patient serum	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay system uses flex-vinyl microtiter plates on which bovine methyl albumin , the respective polynucleotide , a 1 : 80 dilution of patient serum , and tritiated high affinity anti-IgG , - IgA , or - IgM are layered .
	manualset3
141946	7	408815	5	NULL	NULL	0	NULL	high affinity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay system uses flex-vinyl microtiter plates on which bovine methyl albumin , the respective polynucleotide , a 1 : 80 dilution of patient serum , and tritiated high affinity anti-IgG , - IgA , or - IgM are layered .
	manualset3
141947	8	408815	5	NULL	NULL	0	NULL	anti-IgG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay system uses flex-vinyl microtiter plates on which bovine methyl albumin , the respective polynucleotide , a 1 : 80 dilution of patient serum , and tritiated high affinity anti-IgG , - IgA , or - IgM are layered .
	manualset3
141948	9	408815	5	NULL	NULL	0	NULL	anti-IgA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay system uses flex-vinyl microtiter plates on which bovine methyl albumin , the respective polynucleotide , a 1 : 80 dilution of patient serum , and tritiated high affinity anti-IgG , - IgA , or - IgM are layered .
	manualset3
141949	10	408815	5	NULL	NULL	0	NULL	anti-IgM	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay system uses flex-vinyl microtiter plates on which bovine methyl albumin , the respective polynucleotide , a 1 : 80 dilution of patient serum , and tritiated high affinity anti-IgG , - IgA , or - IgM are layered .
	manualset3
141950	1	408816	5	NULL	NULL	0	NULL	assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay was applied for screening of a chemical library consisting of ~ 27 , 000 compounds and proved to be highly reliable ( average Z ' factor of 0.89 ) .
	manualset3
141951	2	408816	5	NULL	NULL	0	NULL	screening	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay was applied for screening of a chemical library consisting of ~ 27 , 000 compounds and proved to be highly reliable ( average Z ' factor of 0.89 ) .
	manualset3
141952	3	408816	5	NULL	NULL	0	NULL	 chemical library 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay was applied for screening of a chemical library consisting of ~ 27 , 000 compounds and proved to be highly reliable ( average Z ' factor of 0.89 ) .
	manualset3
141953	4	408816	5	NULL	NULL	0	NULL	~ 27 , 000 compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay was applied for screening of a chemical library consisting of ~ 27 , 000 compounds and proved to be highly reliable ( average Z ' factor of 0.89 ) .
	manualset3
141954	5	408816	5	NULL	NULL	0	NULL	 average Z ' factor	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay was applied for screening of a chemical library consisting of ~ 27 , 000 compounds and proved to be highly reliable ( average Z ' factor of 0.89 ) .
	manualset3
141955	6	408816	5	NULL	NULL	0	NULL	0.89	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay was applied for screening of a chemical library consisting of ~ 27 , 000 compounds and proved to be highly reliable ( average Z ' factor of 0.89 ) .
	manualset3
141956	1	408817	5	NULL	NULL	0	NULL	assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay was positive in 30 patients , 11 of whom had a definite cardiac diagnosis ( acute myocardial infarction in 4 and unstable angina pectoris in 7 ) .
	manualset3
141957	2	408817	5	NULL	NULL	0	NULL	30 patients	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay was positive in 30 patients , 11 of whom had a definite cardiac diagnosis ( acute myocardial infarction in 4 and unstable angina pectoris in 7 ) .
	manualset3
141958	3	408817	5	NULL	NULL	0	NULL	11	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay was positive in 30 patients , 11 of whom had a definite cardiac diagnosis ( acute myocardial infarction in 4 and unstable angina pectoris in 7 ) .
	manualset3
141959	4	408817	5	NULL	NULL	0	NULL	definite cardiac diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay was positive in 30 patients , 11 of whom had a definite cardiac diagnosis ( acute myocardial infarction in 4 and unstable angina pectoris in 7 ) .
	manualset3
141960	5	408817	5	NULL	NULL	0	NULL	acute myocardial infarction	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay was positive in 30 patients , 11 of whom had a definite cardiac diagnosis ( acute myocardial infarction in 4 and unstable angina pectoris in 7 ) .
	manualset3
141961	6	408817	5	NULL	NULL	0	NULL	 4	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay was positive in 30 patients , 11 of whom had a definite cardiac diagnosis ( acute myocardial infarction in 4 and unstable angina pectoris in 7 ) .
	manualset3
141962	7	408817	5	NULL	NULL	0	NULL	unstable angina pectoris	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay was positive in 30 patients , 11 of whom had a definite cardiac diagnosis ( acute myocardial infarction in 4 and unstable angina pectoris in 7 ) .
	manualset3
141963	8	408817	5	NULL	NULL	0	NULL	7	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay was positive in 30 patients , 11 of whom had a definite cardiac diagnosis ( acute myocardial infarction in 4 and unstable angina pectoris in 7 ) .
	manualset3
141964	1	408818	5	NULL	NULL	0	NULL	assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay was used to detect TB infection by incubating whole blood overnight with human , avian , and bovine tuberculin purified protein derivatives ( PPDs ) , as well as positive ( mitogen ) - and negative-control preparations .
	manualset3
141965	2	408818	5	NULL	NULL	0	NULL	TB infection	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay was used to detect TB infection by incubating whole blood overnight with human , avian , and bovine tuberculin purified protein derivatives ( PPDs ) , as well as positive ( mitogen ) - and negative-control preparations .
	manualset3
141966	3	408818	5	NULL	NULL	0	NULL	whole blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay was used to detect TB infection by incubating whole blood overnight with human , avian , and bovine tuberculin purified protein derivatives ( PPDs ) , as well as positive ( mitogen ) - and negative-control preparations .
	manualset3
141967	4	408818	5	NULL	NULL	0	NULL	overnight	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay was used to detect TB infection by incubating whole blood overnight with human , avian , and bovine tuberculin purified protein derivatives ( PPDs ) , as well as positive ( mitogen ) - and negative-control preparations .
	manualset3
141968	5	408818	5	NULL	NULL	0	NULL	human tuberculin purified protein derivatives ( PPDs )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay was used to detect TB infection by incubating whole blood overnight with human , avian , and bovine tuberculin purified protein derivatives ( PPDs ) , as well as positive ( mitogen ) - and negative-control preparations .
	manualset3
141969	6	408818	5	NULL	NULL	0	NULL	avian tuberculin purified protein derivatives ( PPDs )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay was used to detect TB infection by incubating whole blood overnight with human , avian , and bovine tuberculin purified protein derivatives ( PPDs ) , as well as positive ( mitogen ) - and negative-control preparations .
	manualset3
141970	7	408818	5	NULL	NULL	0	NULL	bovine tuberculin purified protein derivatives ( PPDs )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay was used to detect TB infection by incubating whole blood overnight with human , avian , and bovine tuberculin purified protein derivatives ( PPDs ) , as well as positive ( mitogen ) - and negative-control preparations .
	manualset3
141971	8	408818	5	NULL	NULL	0	NULL	positive ( mitogen ) - control preparations	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay was used to detect TB infection by incubating whole blood overnight with human , avian , and bovine tuberculin purified protein derivatives ( PPDs ) , as well as positive ( mitogen ) - and negative-control preparations .
	manualset3
141972	9	408818	5	NULL	NULL	0	NULL	negative-control preparations	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The assay was used to detect TB infection by incubating whole blood overnight with human , avian , and bovine tuberculin purified protein derivatives ( PPDs ) , as well as positive ( mitogen ) - and negative-control preparations .
	manualset3
141973	1	408819	5	NULL	NULL	0	NULL	association	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The association between antipsychotic agents and the risk of myocardial infarction : a systematic review .
	manualset3
141974	2	408819	5	NULL	NULL	0	NULL	antipsychotic agents	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The association between antipsychotic agents and the risk of myocardial infarction : a systematic review .
	manualset3
141975	3	408819	5	NULL	NULL	0	NULL	risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The association between antipsychotic agents and the risk of myocardial infarction : a systematic review .
	manualset3
141976	4	408819	5	NULL	NULL	0	NULL	myocardial infarction	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The association between antipsychotic agents and the risk of myocardial infarction : a systematic review .
	manualset3
141977	5	408819	5	NULL	NULL	0	NULL	systematic review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The association between antipsychotic agents and the risk of myocardial infarction : a systematic review .
	manualset3
141978	1	408820	5	NULL	NULL	0	NULL	association	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The association between celiac disease ( CD ) and primary biliary cirrhosis ( PBC ) has been reported in literature .
	manualset3
141979	2	408820	5	NULL	NULL	0	NULL	celiac disease ( CD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The association between celiac disease ( CD ) and primary biliary cirrhosis ( PBC ) has been reported in literature .
	manualset3
141980	3	408820	5	NULL	NULL	0	NULL	primary biliary cirrhosis ( PBC ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The association between celiac disease ( CD ) and primary biliary cirrhosis ( PBC ) has been reported in literature .
	manualset3
141981	4	408820	5	NULL	NULL	0	NULL	literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The association between celiac disease ( CD ) and primary biliary cirrhosis ( PBC ) has been reported in literature .
	manualset3
141982	1	408821	5	NULL	NULL	0	NULL	association	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The association between total hip arthroplasty and malignancy is discussed , as well as its frequency worldwide .
	manualset3
141983	2	408821	5	NULL	NULL	0	NULL	total hip arthroplasty	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The association between total hip arthroplasty and malignancy is discussed , as well as its frequency worldwide .
	manualset3
141984	3	408821	5	NULL	NULL	0	NULL	malignancy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The association between total hip arthroplasty and malignancy is discussed , as well as its frequency worldwide .
	manualset3
141985	4	408821	5	NULL	NULL	0	NULL	frequency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The association between total hip arthroplasty and malignancy is discussed , as well as its frequency worldwide .
	manualset3
141986	5	408821	5	NULL	NULL	0	NULL	worldwide	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The association between total hip arthroplasty and malignancy is discussed , as well as its frequency worldwide .
	manualset3
141987	1	408822	5	NULL	NULL	0	NULL	association	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The association of dietary/serum measures of vitamin D status with HNC recurrence , second primary cancer ( SPC ) incidence , and overall mortality was evaluated using multivariate Cox proportional hazard models .
	manualset3
141988	2	408822	5	NULL	NULL	0	NULL	dietary/serum measures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The association of dietary/serum measures of vitamin D status with HNC recurrence , second primary cancer ( SPC ) incidence , and overall mortality was evaluated using multivariate Cox proportional hazard models .
	manualset3
141989	3	408822	5	NULL	NULL	0	NULL	vitamin D status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The association of dietary/serum measures of vitamin D status with HNC recurrence , second primary cancer ( SPC ) incidence , and overall mortality was evaluated using multivariate Cox proportional hazard models .
	manualset3
141990	4	408822	5	NULL	NULL	0	NULL	HNC recurrence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The association of dietary/serum measures of vitamin D status with HNC recurrence , second primary cancer ( SPC ) incidence , and overall mortality was evaluated using multivariate Cox proportional hazard models .
	manualset3
141991	5	408822	5	NULL	NULL	0	NULL	second primary cancer ( SPC ) incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The association of dietary/serum measures of vitamin D status with HNC recurrence , second primary cancer ( SPC ) incidence , and overall mortality was evaluated using multivariate Cox proportional hazard models .
	manualset3
141992	6	408822	5	NULL	NULL	0	NULL	mortality	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The association of dietary/serum measures of vitamin D status with HNC recurrence , second primary cancer ( SPC ) incidence , and overall mortality was evaluated using multivariate Cox proportional hazard models .
	manualset3
141993	7	408822	5	NULL	NULL	0	NULL	multivariate Cox proportional hazard models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The association of dietary/serum measures of vitamin D status with HNC recurrence , second primary cancer ( SPC ) incidence , and overall mortality was evaluated using multivariate Cox proportional hazard models .
	manualset3
141994	1	408823	5	NULL	NULL	0	NULL	association	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The association of fibrinogen with the surface of the platelets was visualized using an electron microscope immunocytochemical method .
	manualset3
141995	2	408823	5	NULL	NULL	0	NULL	fibrinogen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The association of fibrinogen with the surface of the platelets was visualized using an electron microscope immunocytochemical method .
	manualset3
141996	3	408823	5	NULL	NULL	0	NULL	surface	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The association of fibrinogen with the surface of the platelets was visualized using an electron microscope immunocytochemical method .
	manualset3
141997	4	408823	5	NULL	NULL	0	NULL	platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The association of fibrinogen with the surface of the platelets was visualized using an electron microscope immunocytochemical method .
	manualset3
141998	5	408823	5	NULL	NULL	0	NULL	electron microscope immunocytochemical method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The association of fibrinogen with the surface of the platelets was visualized using an electron microscope immunocytochemical method .
	manualset3
141999	1	408824	5	NULL	NULL	0	NULL	association	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The association of macular rash , pruritus , low platelet count and leukopenia was statistically predictive of dengue but not clinically , since these four signs occur in many other viral infections .
	manualset3
142000	2	408824	5	NULL	NULL	0	NULL	macular rash	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The association of macular rash , pruritus , low platelet count and leukopenia was statistically predictive of dengue but not clinically , since these four signs occur in many other viral infections .
	manualset3
142001	3	408824	5	NULL	NULL	NULL	NULL	pruritus	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The association of macular rash , pruritus , low platelet count and leukopenia was statistically predictive of dengue but not clinically , since these four signs occur in many other viral infections .
	manualset3
142002	4	408824	5	NULL	NULL	0	NULL	low platelet count	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The association of macular rash , pruritus , low platelet count and leukopenia was statistically predictive of dengue but not clinically , since these four signs occur in many other viral infections .
	manualset3
142003	5	408824	5	NULL	NULL	0	NULL	leukopenia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The association of macular rash , pruritus , low platelet count and leukopenia was statistically predictive of dengue but not clinically , since these four signs occur in many other viral infections .
	manualset3
142004	6	408824	5	NULL	NULL	0	NULL	dengue	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The association of macular rash , pruritus , low platelet count and leukopenia was statistically predictive of dengue but not clinically , since these four signs occur in many other viral infections .
	manualset3
142005	7	408824	5	NULL	NULL	0	NULL	four signs 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The association of macular rash , pruritus , low platelet count and leukopenia was statistically predictive of dengue but not clinically , since these four signs occur in many other viral infections .
	manualset3
142006	8	408824	5	NULL	NULL	0	NULL	 viral infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The association of macular rash , pruritus , low platelet count and leukopenia was statistically predictive of dengue but not clinically , since these four signs occur in many other viral infections .
	manualset3
142007	1	408825	5	NULL	NULL	0	NULL	scenario	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A scenario of the origin of the genetic apparatus is described where the surface and physico-chemical properties of lipid bilayers and multilayers of vesicles play a crucial role .
	manualset3
142008	2	408825	5	NULL	NULL	0	NULL	origin	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A scenario of the origin of the genetic apparatus is described where the surface and physico-chemical properties of lipid bilayers and multilayers of vesicles play a crucial role .
	manualset3
142009	3	408825	5	NULL	NULL	0	NULL	genetic apparatus	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A scenario of the origin of the genetic apparatus is described where the surface and physico-chemical properties of lipid bilayers and multilayers of vesicles play a crucial role .
	manualset3
142010	4	408825	5	NULL	NULL	0	NULL	surface of lipid bilayers	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A scenario of the origin of the genetic apparatus is described where the surface and physico-chemical properties of lipid bilayers and multilayers of vesicles play a crucial role .
	manualset3
142011	5	408825	5	NULL	NULL	0	NULL	physico-chemical properties of lipid bilayers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A scenario of the origin of the genetic apparatus is described where the surface and physico-chemical properties of lipid bilayers and multilayers of vesicles play a crucial role .
	manualset3
142012	6	408825	5	NULL	NULL	0	NULL	multilayers	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A scenario of the origin of the genetic apparatus is described where the surface and physico-chemical properties of lipid bilayers and multilayers of vesicles play a crucial role .
	manualset3
142013	7	408825	5	NULL	NULL	0	NULL	vesicles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A scenario of the origin of the genetic apparatus is described where the surface and physico-chemical properties of lipid bilayers and multilayers of vesicles play a crucial role .
	manualset3
142014	8	408825	5	NULL	NULL	0	NULL	crucial role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A scenario of the origin of the genetic apparatus is described where the surface and physico-chemical properties of lipid bilayers and multilayers of vesicles play a crucial role .
	manualset3
142015	1	408826	5	NULL	NULL	0	NULL	associative interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The associative interaction leads to the formation of ionic pairs .
	manualset3
142016	2	408826	5	NULL	NULL	0	NULL	formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The associative interaction leads to the formation of ionic pairs .
	manualset3
142017	3	408826	5	NULL	NULL	0	NULL	ionic pairs	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The associative interaction leads to the formation of ionic pairs .
	manualset3
142018	1	408827	5	NULL	NULL	0	NULL	asthenia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The asthenia usually reported by these patients is due to depression and should not be blamed on deficiency of the adrenal cortex .
	manualset3
142019	2	408827	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The asthenia usually reported by these patients is due to depression and should not be blamed on deficiency of the adrenal cortex .
	manualset3
142020	3	408827	5	NULL	NULL	0	NULL	depression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The asthenia usually reported by these patients is due to depression and should not be blamed on deficiency of the adrenal cortex .
	manualset3
142021	4	408827	5	NULL	NULL	0	NULL	deficiency of the adrenal cortex	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The asthenia usually reported by these patients is due to depression and should not be blamed on deficiency of the adrenal cortex .
	manualset3
142022	1	408828	5	NULL	NULL	0	NULL	attachment	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The attachment may be sterilized by soaking .
	manualset3
142023	1	408829	5	NULL	NULL	0	NULL	attachment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The attachment of tendons , ligaments , and joint capsule to bone ( entheses ) is reviewed and new options for visualizing key components of entheses provided by ultrashort TE ( UTE ) pulse sequences are described .
	manualset3
142024	2	408829	5	NULL	NULL	0	NULL	tendons	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The attachment of tendons , ligaments , and joint capsule to bone ( entheses ) is reviewed and new options for visualizing key components of entheses provided by ultrashort TE ( UTE ) pulse sequences are described .
	manualset3
142025	3	408829	5	NULL	NULL	0	NULL	ligaments	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The attachment of tendons , ligaments , and joint capsule to bone ( entheses ) is reviewed and new options for visualizing key components of entheses provided by ultrashort TE ( UTE ) pulse sequences are described .
	manualset3
142026	4	408829	5	NULL	NULL	0	NULL	joint capsule	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The attachment of tendons , ligaments , and joint capsule to bone ( entheses ) is reviewed and new options for visualizing key components of entheses provided by ultrashort TE ( UTE ) pulse sequences are described .
	manualset3
142027	5	408829	5	NULL	NULL	0	NULL	bone ( entheses )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The attachment of tendons , ligaments , and joint capsule to bone ( entheses ) is reviewed and new options for visualizing key components of entheses provided by ultrashort TE ( UTE ) pulse sequences are described .
	manualset3
142028	6	408829	5	NULL	NULL	0	NULL	options	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The attachment of tendons , ligaments , and joint capsule to bone ( entheses ) is reviewed and new options for visualizing key components of entheses provided by ultrashort TE ( UTE ) pulse sequences are described .
	manualset3
142029	7	408829	5	NULL	NULL	0	NULL	key components 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The attachment of tendons , ligaments , and joint capsule to bone ( entheses ) is reviewed and new options for visualizing key components of entheses provided by ultrashort TE ( UTE ) pulse sequences are described .
	manualset3
142030	8	408829	5	NULL	NULL	0	NULL	entheses	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The attachment of tendons , ligaments , and joint capsule to bone ( entheses ) is reviewed and new options for visualizing key components of entheses provided by ultrashort TE ( UTE ) pulse sequences are described .
	manualset3
142031	9	408829	5	NULL	NULL	0	NULL	ultrashort TE ( UTE ) pulse sequences	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The attachment of tendons , ligaments , and joint capsule to bone ( entheses ) is reviewed and new options for visualizing key components of entheses provided by ultrashort TE ( UTE ) pulse sequences are described .
	manualset3
142032	1	408830	5	NULL	NULL	0	NULL	attachment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The attachment of the GPI moiety to the carboxyl-terminus after proteolytic cleavage of a C-terminal propeptide is performed by the transamidase complex .
	manualset3
142033	2	408830	5	NULL	NULL	0	NULL	GPI moiety	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The attachment of the GPI moiety to the carboxyl-terminus after proteolytic cleavage of a C-terminal propeptide is performed by the transamidase complex .
	manualset3
142034	3	408830	5	NULL	NULL	0	NULL	carboxyl-terminus 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The attachment of the GPI moiety to the carboxyl-terminus after proteolytic cleavage of a C-terminal propeptide is performed by the transamidase complex .
	manualset3
142035	4	408830	5	NULL	NULL	0	NULL	proteolytic cleavage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The attachment of the GPI moiety to the carboxyl-terminus after proteolytic cleavage of a C-terminal propeptide is performed by the transamidase complex .
	manualset3
142036	5	408830	5	NULL	NULL	0	NULL	C-terminal propeptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The attachment of the GPI moiety to the carboxyl-terminus after proteolytic cleavage of a C-terminal propeptide is performed by the transamidase complex .
	manualset3
142037	6	408830	5	NULL	NULL	0	NULL	transamidase complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The attachment of the GPI moiety to the carboxyl-terminus after proteolytic cleavage of a C-terminal propeptide is performed by the transamidase complex .
	manualset3
142038	1	408831	5	NULL	NULL	0	NULL	attachment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The attachment of transfected cells to microcarrier beads enabled the efficient production of large quantities of rLCAT in a serum-free medium .
	manualset3
142039	2	408831	5	NULL	NULL	0	NULL	transfected cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The attachment of transfected cells to microcarrier beads enabled the efficient production of large quantities of rLCAT in a serum-free medium .
	manualset3
142040	3	408831	5	NULL	NULL	0	NULL	microcarrier beads	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The attachment of transfected cells to microcarrier beads enabled the efficient production of large quantities of rLCAT in a serum-free medium .
	manualset3
142041	4	408831	5	NULL	NULL	0	NULL	production 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The attachment of transfected cells to microcarrier beads enabled the efficient production of large quantities of rLCAT in a serum-free medium .
	manualset3
142042	5	408831	5	NULL	NULL	0	NULL	large quantities 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The attachment of transfected cells to microcarrier beads enabled the efficient production of large quantities of rLCAT in a serum-free medium .
	manualset3
142043	6	408831	5	NULL	NULL	0	NULL	rLCAT	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The attachment of transfected cells to microcarrier beads enabled the efficient production of large quantities of rLCAT in a serum-free medium .
	manualset3
142044	7	408831	5	NULL	NULL	0	NULL	serum-free medium 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The attachment of transfected cells to microcarrier beads enabled the efficient production of large quantities of rLCAT in a serum-free medium .
	manualset3
142045	1	408832	5	NULL	NULL	0	NULL	attenuation of vision	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The attenuation of vision that has long been known to accompany saccadic eye movement has a significant component that is not attributable to visual masking or image smear , and this suppression of vision is now associated with nonsaccadic movement .
	manualset3
142046	2	408832	5	NULL	NULL	0	NULL	saccadic eye movement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The attenuation of vision that has long been known to accompany saccadic eye movement has a significant component that is not attributable to visual masking or image smear , and this suppression of vision is now associated with nonsaccadic movement .
	manualset3
142047	3	408832	5	NULL	NULL	0	NULL	significant component	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The attenuation of vision that has long been known to accompany saccadic eye movement has a significant component that is not attributable to visual masking or image smear , and this suppression of vision is now associated with nonsaccadic movement .
	manualset3
142048	4	408832	5	NULL	NULL	0	NULL	visual masking or image smear	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The attenuation of vision that has long been known to accompany saccadic eye movement has a significant component that is not attributable to visual masking or image smear , and this suppression of vision is now associated with nonsaccadic movement .
	manualset3
142049	5	408832	5	NULL	NULL	0	NULL	suppression of vision	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The attenuation of vision that has long been known to accompany saccadic eye movement has a significant component that is not attributable to visual masking or image smear , and this suppression of vision is now associated with nonsaccadic movement .
	manualset3
142050	6	408832	5	NULL	NULL	0	NULL	nonsaccadic movement 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The attenuation of vision that has long been known to accompany saccadic eye movement has a significant component that is not attributable to visual masking or image smear , and this suppression of vision is now associated with nonsaccadic movement .
	manualset3
142051	1	408833	5	NULL	NULL	0	NULL	attestations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The attestations , required under the Immigration and Nationality Act , pertain to substantial disruption in the delivery of health care services , absence of adverse effect on wages and working conditions of similarly employed registered nurses , payment of wages to nonimmigrant alien nurses employed by the facility at wage rates paid to other registered nurses similarly employed by the facility , taking timely and significant steps designed to recruit and retain U.S. nurses in order to reduce dependence on nonimmigrant alien nurses , absence of a strike or lockout , and giving appropriate notice of filing .
	manualset3
142052	2	408833	5	NULL	NULL	0	NULL	Immigration and Nationality Act	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The attestations , required under the Immigration and Nationality Act , pertain to substantial disruption in the delivery of health care services , absence of adverse effect on wages and working conditions of similarly employed registered nurses , payment of wages to nonimmigrant alien nurses employed by the facility at wage rates paid to other registered nurses similarly employed by the facility , taking timely and significant steps designed to recruit and retain U.S. nurses in order to reduce dependence on nonimmigrant alien nurses , absence of a strike or lockout , and giving appropriate notice of filing .
	manualset3
142053	3	408833	5	NULL	NULL	0	NULL	disruption 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The attestations , required under the Immigration and Nationality Act , pertain to substantial disruption in the delivery of health care services , absence of adverse effect on wages and working conditions of similarly employed registered nurses , payment of wages to nonimmigrant alien nurses employed by the facility at wage rates paid to other registered nurses similarly employed by the facility , taking timely and significant steps designed to recruit and retain U.S. nurses in order to reduce dependence on nonimmigrant alien nurses , absence of a strike or lockout , and giving appropriate notice of filing .
	manualset3
142054	4	408833	5	NULL	NULL	0	NULL	delivery 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The attestations , required under the Immigration and Nationality Act , pertain to substantial disruption in the delivery of health care services , absence of adverse effect on wages and working conditions of similarly employed registered nurses , payment of wages to nonimmigrant alien nurses employed by the facility at wage rates paid to other registered nurses similarly employed by the facility , taking timely and significant steps designed to recruit and retain U.S. nurses in order to reduce dependence on nonimmigrant alien nurses , absence of a strike or lockout , and giving appropriate notice of filing .
	manualset3
142055	5	408833	5	NULL	NULL	0	NULL	health care services 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The attestations , required under the Immigration and Nationality Act , pertain to substantial disruption in the delivery of health care services , absence of adverse effect on wages and working conditions of similarly employed registered nurses , payment of wages to nonimmigrant alien nurses employed by the facility at wage rates paid to other registered nurses similarly employed by the facility , taking timely and significant steps designed to recruit and retain U.S. nurses in order to reduce dependence on nonimmigrant alien nurses , absence of a strike or lockout , and giving appropriate notice of filing .
	manualset3
142056	6	408833	5	NULL	NULL	0	NULL	absence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The attestations , required under the Immigration and Nationality Act , pertain to substantial disruption in the delivery of health care services , absence of adverse effect on wages and working conditions of similarly employed registered nurses , payment of wages to nonimmigrant alien nurses employed by the facility at wage rates paid to other registered nurses similarly employed by the facility , taking timely and significant steps designed to recruit and retain U.S. nurses in order to reduce dependence on nonimmigrant alien nurses , absence of a strike or lockout , and giving appropriate notice of filing .
	manualset3
142057	7	408833	5	NULL	NULL	0	NULL	adverse effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The attestations , required under the Immigration and Nationality Act , pertain to substantial disruption in the delivery of health care services , absence of adverse effect on wages and working conditions of similarly employed registered nurses , payment of wages to nonimmigrant alien nurses employed by the facility at wage rates paid to other registered nurses similarly employed by the facility , taking timely and significant steps designed to recruit and retain U.S. nurses in order to reduce dependence on nonimmigrant alien nurses , absence of a strike or lockout , and giving appropriate notice of filing .
	manualset3
142058	8	408833	5	NULL	NULL	0	NULL	wages 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The attestations , required under the Immigration and Nationality Act , pertain to substantial disruption in the delivery of health care services , absence of adverse effect on wages and working conditions of similarly employed registered nurses , payment of wages to nonimmigrant alien nurses employed by the facility at wage rates paid to other registered nurses similarly employed by the facility , taking timely and significant steps designed to recruit and retain U.S. nurses in order to reduce dependence on nonimmigrant alien nurses , absence of a strike or lockout , and giving appropriate notice of filing .
	manualset3
142059	9	408833	5	NULL	NULL	0	NULL	working conditions	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The attestations , required under the Immigration and Nationality Act , pertain to substantial disruption in the delivery of health care services , absence of adverse effect on wages and working conditions of similarly employed registered nurses , payment of wages to nonimmigrant alien nurses employed by the facility at wage rates paid to other registered nurses similarly employed by the facility , taking timely and significant steps designed to recruit and retain U.S. nurses in order to reduce dependence on nonimmigrant alien nurses , absence of a strike or lockout , and giving appropriate notice of filing .
	manualset3
142060	10	408833	5	NULL	NULL	0	NULL	registered nurses 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The attestations , required under the Immigration and Nationality Act , pertain to substantial disruption in the delivery of health care services , absence of adverse effect on wages and working conditions of similarly employed registered nurses , payment of wages to nonimmigrant alien nurses employed by the facility at wage rates paid to other registered nurses similarly employed by the facility , taking timely and significant steps designed to recruit and retain U.S. nurses in order to reduce dependence on nonimmigrant alien nurses , absence of a strike or lockout , and giving appropriate notice of filing .
	manualset3
142061	11	408833	5	NULL	NULL	0	NULL	payment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The attestations , required under the Immigration and Nationality Act , pertain to substantial disruption in the delivery of health care services , absence of adverse effect on wages and working conditions of similarly employed registered nurses , payment of wages to nonimmigrant alien nurses employed by the facility at wage rates paid to other registered nurses similarly employed by the facility , taking timely and significant steps designed to recruit and retain U.S. nurses in order to reduce dependence on nonimmigrant alien nurses , absence of a strike or lockout , and giving appropriate notice of filing .
	manualset3
142062	12	408833	5	NULL	NULL	0	NULL	wages 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The attestations , required under the Immigration and Nationality Act , pertain to substantial disruption in the delivery of health care services , absence of adverse effect on wages and working conditions of similarly employed registered nurses , payment of wages to nonimmigrant alien nurses employed by the facility at wage rates paid to other registered nurses similarly employed by the facility , taking timely and significant steps designed to recruit and retain U.S. nurses in order to reduce dependence on nonimmigrant alien nurses , absence of a strike or lockout , and giving appropriate notice of filing .
	manualset3
142063	13	408833	5	NULL	NULL	0	NULL	nonimmigrant alien nurses	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The attestations , required under the Immigration and Nationality Act , pertain to substantial disruption in the delivery of health care services , absence of adverse effect on wages and working conditions of similarly employed registered nurses , payment of wages to nonimmigrant alien nurses employed by the facility at wage rates paid to other registered nurses similarly employed by the facility , taking timely and significant steps designed to recruit and retain U.S. nurses in order to reduce dependence on nonimmigrant alien nurses , absence of a strike or lockout , and giving appropriate notice of filing .
	manualset3
142064	14	408833	5	NULL	NULL	0	NULL	facility 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The attestations , required under the Immigration and Nationality Act , pertain to substantial disruption in the delivery of health care services , absence of adverse effect on wages and working conditions of similarly employed registered nurses , payment of wages to nonimmigrant alien nurses employed by the facility at wage rates paid to other registered nurses similarly employed by the facility , taking timely and significant steps designed to recruit and retain U.S. nurses in order to reduce dependence on nonimmigrant alien nurses , absence of a strike or lockout , and giving appropriate notice of filing .
	manualset3
142065	15	408833	5	NULL	NULL	0	NULL	wage rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The attestations , required under the Immigration and Nationality Act , pertain to substantial disruption in the delivery of health care services , absence of adverse effect on wages and working conditions of similarly employed registered nurses , payment of wages to nonimmigrant alien nurses employed by the facility at wage rates paid to other registered nurses similarly employed by the facility , taking timely and significant steps designed to recruit and retain U.S. nurses in order to reduce dependence on nonimmigrant alien nurses , absence of a strike or lockout , and giving appropriate notice of filing .
	manualset3
142066	16	408833	5	NULL	NULL	0	NULL	registered nurses	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The attestations , required under the Immigration and Nationality Act , pertain to substantial disruption in the delivery of health care services , absence of adverse effect on wages and working conditions of similarly employed registered nurses , payment of wages to nonimmigrant alien nurses employed by the facility at wage rates paid to other registered nurses similarly employed by the facility , taking timely and significant steps designed to recruit and retain U.S. nurses in order to reduce dependence on nonimmigrant alien nurses , absence of a strike or lockout , and giving appropriate notice of filing .
	manualset3
142067	17	408833	5	NULL	NULL	0	NULL	facility 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The attestations , required under the Immigration and Nationality Act , pertain to substantial disruption in the delivery of health care services , absence of adverse effect on wages and working conditions of similarly employed registered nurses , payment of wages to nonimmigrant alien nurses employed by the facility at wage rates paid to other registered nurses similarly employed by the facility , taking timely and significant steps designed to recruit and retain U.S. nurses in order to reduce dependence on nonimmigrant alien nurses , absence of a strike or lockout , and giving appropriate notice of filing .
	manualset3
142068	18	408833	5	NULL	NULL	0	NULL	U.S. nurses	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The attestations , required under the Immigration and Nationality Act , pertain to substantial disruption in the delivery of health care services , absence of adverse effect on wages and working conditions of similarly employed registered nurses , payment of wages to nonimmigrant alien nurses employed by the facility at wage rates paid to other registered nurses similarly employed by the facility , taking timely and significant steps designed to recruit and retain U.S. nurses in order to reduce dependence on nonimmigrant alien nurses , absence of a strike or lockout , and giving appropriate notice of filing .
	manualset3
142069	19	408833	5	NULL	NULL	0	NULL	dependence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The attestations , required under the Immigration and Nationality Act , pertain to substantial disruption in the delivery of health care services , absence of adverse effect on wages and working conditions of similarly employed registered nurses , payment of wages to nonimmigrant alien nurses employed by the facility at wage rates paid to other registered nurses similarly employed by the facility , taking timely and significant steps designed to recruit and retain U.S. nurses in order to reduce dependence on nonimmigrant alien nurses , absence of a strike or lockout , and giving appropriate notice of filing .
	manualset3
142070	20	408833	5	NULL	NULL	0	NULL	nonimmigrant alien nurses	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The attestations , required under the Immigration and Nationality Act , pertain to substantial disruption in the delivery of health care services , absence of adverse effect on wages and working conditions of similarly employed registered nurses , payment of wages to nonimmigrant alien nurses employed by the facility at wage rates paid to other registered nurses similarly employed by the facility , taking timely and significant steps designed to recruit and retain U.S. nurses in order to reduce dependence on nonimmigrant alien nurses , absence of a strike or lockout , and giving appropriate notice of filing .
	manualset3
142071	21	408833	5	NULL	NULL	0	NULL	absence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The attestations , required under the Immigration and Nationality Act , pertain to substantial disruption in the delivery of health care services , absence of adverse effect on wages and working conditions of similarly employed registered nurses , payment of wages to nonimmigrant alien nurses employed by the facility at wage rates paid to other registered nurses similarly employed by the facility , taking timely and significant steps designed to recruit and retain U.S. nurses in order to reduce dependence on nonimmigrant alien nurses , absence of a strike or lockout , and giving appropriate notice of filing .
	manualset3
142072	22	408833	5	NULL	NULL	0	NULL	strike or lockout	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The attestations , required under the Immigration and Nationality Act , pertain to substantial disruption in the delivery of health care services , absence of adverse effect on wages and working conditions of similarly employed registered nurses , payment of wages to nonimmigrant alien nurses employed by the facility at wage rates paid to other registered nurses similarly employed by the facility , taking timely and significant steps designed to recruit and retain U.S. nurses in order to reduce dependence on nonimmigrant alien nurses , absence of a strike or lockout , and giving appropriate notice of filing .
	manualset3
142073	23	408833	5	NULL	NULL	0	NULL	appropriate notice	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The attestations , required under the Immigration and Nationality Act , pertain to substantial disruption in the delivery of health care services , absence of adverse effect on wages and working conditions of similarly employed registered nurses , payment of wages to nonimmigrant alien nurses employed by the facility at wage rates paid to other registered nurses similarly employed by the facility , taking timely and significant steps designed to recruit and retain U.S. nurses in order to reduce dependence on nonimmigrant alien nurses , absence of a strike or lockout , and giving appropriate notice of filing .
	manualset3
142074	1	408834	5	NULL	NULL	0	NULL	augmentation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The augmentation of intracellular calcium elicited by loperamide in cultured cells was dependent on extracellular calcium and was somewhat resistant to agents ( SKF 96365 , miconazole , clotrimazole , nitrendipine , and trifluoperazine ) that in the absence of loperamide effectively blocked SOC channels .
	manualset3
142075	2	408834	5	NULL	NULL	NULL	NULL	intracellular calcium	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The augmentation of intracellular calcium elicited by loperamide in cultured cells was dependent on extracellular calcium and was somewhat resistant to agents ( SKF 96365 , miconazole , clotrimazole , nitrendipine , and trifluoperazine ) that in the absence of loperamide effectively blocked SOC channels .
	manualset3
142076	3	408834	5	NULL	NULL	0	NULL	loperamide 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The augmentation of intracellular calcium elicited by loperamide in cultured cells was dependent on extracellular calcium and was somewhat resistant to agents ( SKF 96365 , miconazole , clotrimazole , nitrendipine , and trifluoperazine ) that in the absence of loperamide effectively blocked SOC channels .
	manualset3
142077	4	408834	5	NULL	NULL	0	NULL	cultured cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The augmentation of intracellular calcium elicited by loperamide in cultured cells was dependent on extracellular calcium and was somewhat resistant to agents ( SKF 96365 , miconazole , clotrimazole , nitrendipine , and trifluoperazine ) that in the absence of loperamide effectively blocked SOC channels .
	manualset3
142078	5	408834	5	NULL	NULL	0	NULL	extracellular calcium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The augmentation of intracellular calcium elicited by loperamide in cultured cells was dependent on extracellular calcium and was somewhat resistant to agents ( SKF 96365 , miconazole , clotrimazole , nitrendipine , and trifluoperazine ) that in the absence of loperamide effectively blocked SOC channels .
	manualset3
142079	6	408834	5	NULL	NULL	0	NULL	agents 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The augmentation of intracellular calcium elicited by loperamide in cultured cells was dependent on extracellular calcium and was somewhat resistant to agents ( SKF 96365 , miconazole , clotrimazole , nitrendipine , and trifluoperazine ) that in the absence of loperamide effectively blocked SOC channels .
	manualset3
142080	7	408834	5	NULL	NULL	0	NULL	SKF 96365 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The augmentation of intracellular calcium elicited by loperamide in cultured cells was dependent on extracellular calcium and was somewhat resistant to agents ( SKF 96365 , miconazole , clotrimazole , nitrendipine , and trifluoperazine ) that in the absence of loperamide effectively blocked SOC channels .
	manualset3
142081	8	408834	5	NULL	NULL	0	NULL	miconazole 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The augmentation of intracellular calcium elicited by loperamide in cultured cells was dependent on extracellular calcium and was somewhat resistant to agents ( SKF 96365 , miconazole , clotrimazole , nitrendipine , and trifluoperazine ) that in the absence of loperamide effectively blocked SOC channels .
	manualset3
142082	9	408834	5	NULL	NULL	0	NULL	clotrimazole 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The augmentation of intracellular calcium elicited by loperamide in cultured cells was dependent on extracellular calcium and was somewhat resistant to agents ( SKF 96365 , miconazole , clotrimazole , nitrendipine , and trifluoperazine ) that in the absence of loperamide effectively blocked SOC channels .
	manualset3
142083	10	408834	5	NULL	NULL	0	NULL	nitrendipine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The augmentation of intracellular calcium elicited by loperamide in cultured cells was dependent on extracellular calcium and was somewhat resistant to agents ( SKF 96365 , miconazole , clotrimazole , nitrendipine , and trifluoperazine ) that in the absence of loperamide effectively blocked SOC channels .
	manualset3
142084	11	408834	5	NULL	NULL	0	NULL	trifluoperazine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The augmentation of intracellular calcium elicited by loperamide in cultured cells was dependent on extracellular calcium and was somewhat resistant to agents ( SKF 96365 , miconazole , clotrimazole , nitrendipine , and trifluoperazine ) that in the absence of loperamide effectively blocked SOC channels .
	manualset3
142085	12	408834	5	NULL	NULL	0	NULL	absence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The augmentation of intracellular calcium elicited by loperamide in cultured cells was dependent on extracellular calcium and was somewhat resistant to agents ( SKF 96365 , miconazole , clotrimazole , nitrendipine , and trifluoperazine ) that in the absence of loperamide effectively blocked SOC channels .
	manualset3
142086	13	408834	5	NULL	NULL	0	NULL	loperamide 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The augmentation of intracellular calcium elicited by loperamide in cultured cells was dependent on extracellular calcium and was somewhat resistant to agents ( SKF 96365 , miconazole , clotrimazole , nitrendipine , and trifluoperazine ) that in the absence of loperamide effectively blocked SOC channels .
	manualset3
142087	14	408834	5	NULL	NULL	0	NULL	SOC channels	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The augmentation of intracellular calcium elicited by loperamide in cultured cells was dependent on extracellular calcium and was somewhat resistant to agents ( SKF 96365 , miconazole , clotrimazole , nitrendipine , and trifluoperazine ) that in the absence of loperamide effectively blocked SOC channels .
	manualset3
142088	1	408835	5	NULL	NULL	0	NULL	aurora B kinase inhibitor AZD1152 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The aurora B kinase inhibitor AZD1152 sensitizes cancer cells to fractionated irradiation and induces mitotic catastrophe .
	manualset3
142089	2	408835	5	NULL	NULL	0	NULL	cancer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The aurora B kinase inhibitor AZD1152 sensitizes cancer cells to fractionated irradiation and induces mitotic catastrophe .
	manualset3
142090	3	408835	5	NULL	NULL	0	NULL	fractionated irradiation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aurora B kinase inhibitor AZD1152 sensitizes cancer cells to fractionated irradiation and induces mitotic catastrophe .
	manualset3
142091	4	408835	5	NULL	NULL	0	NULL	mitotic catastrophe 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aurora B kinase inhibitor AZD1152 sensitizes cancer cells to fractionated irradiation and induces mitotic catastrophe .
	manualset3
142092	1	408836	5	NULL	NULL	0	NULL	authentic signal sequence	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The authentic signal sequence of porcine interferon-gamma was substituted with the honeybee melittin ( HBM ) signal sequence , and expressed in insect cells .
	manualset3
142093	2	408836	5	NULL	NULL	0	NULL	porcine interferon-gamma 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The authentic signal sequence of porcine interferon-gamma was substituted with the honeybee melittin ( HBM ) signal sequence , and expressed in insect cells .
	manualset3
142094	3	408836	5	NULL	NULL	0	NULL	honeybee melittin ( HBM ) signal sequence	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The authentic signal sequence of porcine interferon-gamma was substituted with the honeybee melittin ( HBM ) signal sequence , and expressed in insect cells .
	manualset3
142095	4	408836	5	NULL	NULL	0	NULL	insect cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The authentic signal sequence of porcine interferon-gamma was substituted with the honeybee melittin ( HBM ) signal sequence , and expressed in insect cells .
	manualset3
142096	1	408837	5	NULL	NULL	0	NULL	authentic use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authentic use of the therapist 's self is endorsed as mutative in facilitating personality change in the patient .
	manualset3
142097	2	408837	5	NULL	NULL	0	NULL	therapist 's self 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The authentic use of the therapist 's self is endorsed as mutative in facilitating personality change in the patient .
	manualset3
142098	3	408837	5	NULL	NULL	0	NULL	personality change	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authentic use of the therapist 's self is endorsed as mutative in facilitating personality change in the patient .
	manualset3
142099	4	408837	5	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The authentic use of the therapist 's self is endorsed as mutative in facilitating personality change in the patient .
	manualset3
142100	1	408838	5	NULL	NULL	0	NULL	author 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The author , journal , date and country of publication , patient group studied , study type , relevant outcomes , results and study weaknesses were tabulated .
	manualset3
142101	2	408838	5	NULL	NULL	NULL	NULL	journal 	Journal												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The author , journal , date and country of publication , patient group studied , study type , relevant outcomes , results and study weaknesses were tabulated .
	manualset3
142102	3	408838	5	NULL	NULL	0	NULL	date 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	The author , journal , date and country of publication , patient group studied , study type , relevant outcomes , results and study weaknesses were tabulated .
	manualset3
142103	4	408838	5	NULL	NULL	0	NULL	country 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The author , journal , date and country of publication , patient group studied , study type , relevant outcomes , results and study weaknesses were tabulated .
	manualset3
142104	5	408838	5	NULL	NULL	0	NULL	publication 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The author , journal , date and country of publication , patient group studied , study type , relevant outcomes , results and study weaknesses were tabulated .
	manualset3
142105	6	408838	5	NULL	NULL	0	NULL	patient group 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The author , journal , date and country of publication , patient group studied , study type , relevant outcomes , results and study weaknesses were tabulated .
	manualset3
142106	7	408838	5	NULL	NULL	0	NULL	study type	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The author , journal , date and country of publication , patient group studied , study type , relevant outcomes , results and study weaknesses were tabulated .
	manualset3
142107	8	408838	5	NULL	NULL	NULL	NULL	relevant outcomes	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The author , journal , date and country of publication , patient group studied , study type , relevant outcomes , results and study weaknesses were tabulated .
	manualset3
142108	9	408838	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The author , journal , date and country of publication , patient group studied , study type , relevant outcomes , results and study weaknesses were tabulated .
	manualset3
142109	10	408838	5	NULL	NULL	0	NULL	study weaknesses 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The author , journal , date and country of publication , patient group studied , study type , relevant outcomes , results and study weaknesses were tabulated .
	manualset3
142110	1	408839	5	NULL	NULL	0	NULL	author 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The author aims to demonstrate , through a textual analysis of Freud 's work , how the creation of psychoanalysis as a plausible set of understandings of the human mind has a methodological origin that has sometimes been overlooked : in the Greek concept of techne .
	manualset3
142111	2	408839	5	NULL	NULL	0	NULL	textual analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The author aims to demonstrate , through a textual analysis of Freud 's work , how the creation of psychoanalysis as a plausible set of understandings of the human mind has a methodological origin that has sometimes been overlooked : in the Greek concept of techne .
	manualset3
142112	3	408839	5	NULL	NULL	0	NULL	creation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The author aims to demonstrate , through a textual analysis of Freud 's work , how the creation of psychoanalysis as a plausible set of understandings of the human mind has a methodological origin that has sometimes been overlooked : in the Greek concept of techne .
	manualset3
142113	4	408839	5	NULL	NULL	0	NULL	psychoanalysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The author aims to demonstrate , through a textual analysis of Freud 's work , how the creation of psychoanalysis as a plausible set of understandings of the human mind has a methodological origin that has sometimes been overlooked : in the Greek concept of techne .
	manualset3
142114	5	408839	5	NULL	NULL	0	NULL	understandings 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The author aims to demonstrate , through a textual analysis of Freud 's work , how the creation of psychoanalysis as a plausible set of understandings of the human mind has a methodological origin that has sometimes been overlooked : in the Greek concept of techne .
	manualset3
142115	6	408839	5	NULL	NULL	NULL	NULL	human mind 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The author aims to demonstrate , through a textual analysis of Freud 's work , how the creation of psychoanalysis as a plausible set of understandings of the human mind has a methodological origin that has sometimes been overlooked : in the Greek concept of techne .
	manualset3
142116	7	408839	5	NULL	NULL	0	NULL	methodological origin	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The author aims to demonstrate , through a textual analysis of Freud 's work , how the creation of psychoanalysis as a plausible set of understandings of the human mind has a methodological origin that has sometimes been overlooked : in the Greek concept of techne .
	manualset3
142117	8	408839	5	NULL	NULL	0	NULL	Greek concept of techne	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The author aims to demonstrate , through a textual analysis of Freud 's work , how the creation of psychoanalysis as a plausible set of understandings of the human mind has a methodological origin that has sometimes been overlooked : in the Greek concept of techne .
	manualset3
147965	9	408839	5	NULL	NULL	NULL	NULL	Freud 's work	PublicationOrCitation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The author aims to demonstrate , through a textual analysis of Freud 's work , how the creation of psychoanalysis as a plausible set of understandings of the human mind has a methodological origin that has sometimes been overlooked : in the Greek concept of techne .
	manualset3
142118	1	408840	5	NULL	NULL	0	NULL	author 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The author also presents a second scheme , more stylized and resumative which seems to show more clearly the antagonism between hepatic oxidation of FFA ( expressing the catabolic phase ) and aerobic glycolysis ( expressing the anabolic phase ) ; this may partly explain why the two phases can not be simultaneously but only alternatively functional .
	manualset3
142119	2	408840	5	NULL	NULL	0	NULL	second scheme	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The author also presents a second scheme , more stylized and resumative which seems to show more clearly the antagonism between hepatic oxidation of FFA ( expressing the catabolic phase ) and aerobic glycolysis ( expressing the anabolic phase ) ; this may partly explain why the two phases can not be simultaneously but only alternatively functional .
	manualset3
142120	3	408840	5	NULL	NULL	0	NULL	antagonism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The author also presents a second scheme , more stylized and resumative which seems to show more clearly the antagonism between hepatic oxidation of FFA ( expressing the catabolic phase ) and aerobic glycolysis ( expressing the anabolic phase ) ; this may partly explain why the two phases can not be simultaneously but only alternatively functional .
	manualset3
142121	4	408840	5	NULL	NULL	0	NULL	oxidation of FFA 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The author also presents a second scheme , more stylized and resumative which seems to show more clearly the antagonism between hepatic oxidation of FFA ( expressing the catabolic phase ) and aerobic glycolysis ( expressing the anabolic phase ) ; this may partly explain why the two phases can not be simultaneously but only alternatively functional .
	manualset3
142122	5	408840	5	NULL	NULL	0	NULL	catabolic phase	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The author also presents a second scheme , more stylized and resumative which seems to show more clearly the antagonism between hepatic oxidation of FFA ( expressing the catabolic phase ) and aerobic glycolysis ( expressing the anabolic phase ) ; this may partly explain why the two phases can not be simultaneously but only alternatively functional .
	manualset3
142123	6	408840	5	NULL	NULL	0	NULL	aerobic glycolysis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The author also presents a second scheme , more stylized and resumative which seems to show more clearly the antagonism between hepatic oxidation of FFA ( expressing the catabolic phase ) and aerobic glycolysis ( expressing the anabolic phase ) ; this may partly explain why the two phases can not be simultaneously but only alternatively functional .
	manualset3
142124	7	408840	5	NULL	NULL	0	NULL	anabolic phase 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The author also presents a second scheme , more stylized and resumative which seems to show more clearly the antagonism between hepatic oxidation of FFA ( expressing the catabolic phase ) and aerobic glycolysis ( expressing the anabolic phase ) ; this may partly explain why the two phases can not be simultaneously but only alternatively functional .
	manualset3
142125	8	408840	5	NULL	NULL	0	NULL	two phases	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The author also presents a second scheme , more stylized and resumative which seems to show more clearly the antagonism between hepatic oxidation of FFA ( expressing the catabolic phase ) and aerobic glycolysis ( expressing the anabolic phase ) ; this may partly explain why the two phases can not be simultaneously but only alternatively functional .
	manualset3
142126	1	408841	5	NULL	NULL	0	NULL	author 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The author concludes that cascade genetic screening for FH leads to health benefits and is cost-effective without causing psychological or social damage .
	manualset3
142127	2	408841	5	NULL	NULL	0	NULL	cascade genetic screening	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The author concludes that cascade genetic screening for FH leads to health benefits and is cost-effective without causing psychological or social damage .
	manualset3
142128	3	408841	5	NULL	NULL	0	NULL	FH 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The author concludes that cascade genetic screening for FH leads to health benefits and is cost-effective without causing psychological or social damage .
	manualset3
142129	4	408841	5	NULL	NULL	0	NULL	health benefits 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The author concludes that cascade genetic screening for FH leads to health benefits and is cost-effective without causing psychological or social damage .
	manualset3
142130	5	408841	5	NULL	NULL	0	NULL	psychological damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The author concludes that cascade genetic screening for FH leads to health benefits and is cost-effective without causing psychological or social damage .
	manualset3
142131	6	408841	5	NULL	NULL	0	NULL	social damage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The author concludes that cascade genetic screening for FH leads to health benefits and is cost-effective without causing psychological or social damage .
	manualset3
142132	1	408842	5	NULL	NULL	0	NULL	author 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The author considers early cellular inflammation to result from multiple , simultaneous , overlapping , amplifying and inhibitory systems .
	manualset3
142133	2	408842	5	NULL	NULL	0	NULL	early cellular inflammation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The author considers early cellular inflammation to result from multiple , simultaneous , overlapping , amplifying and inhibitory systems .
	manualset3
142134	3	408842	5	NULL	NULL	0	NULL	multiple systems	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The author considers early cellular inflammation to result from multiple , simultaneous , overlapping , amplifying and inhibitory systems .
	manualset3
142135	4	408842	5	NULL	NULL	0	NULL	simultaneous systems	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The author considers early cellular inflammation to result from multiple , simultaneous , overlapping , amplifying and inhibitory systems .
	manualset3
142136	5	408842	5	NULL	NULL	0	NULL	overlapping systems	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The author considers early cellular inflammation to result from multiple , simultaneous , overlapping , amplifying and inhibitory systems .
	manualset3
142137	6	408842	5	NULL	NULL	0	NULL	amplifying systems	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The author considers early cellular inflammation to result from multiple , simultaneous , overlapping , amplifying and inhibitory systems .
	manualset3
142138	7	408842	5	NULL	NULL	0	NULL	inhibitory systems	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The author considers early cellular inflammation to result from multiple , simultaneous , overlapping , amplifying and inhibitory systems .
	manualset3
142139	1	408843	5	NULL	NULL	0	NULL	author 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The author demonstrates the presence of estrogen and progesterone receptors in the trophoblast .
	manualset3
142140	2	408843	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The author demonstrates the presence of estrogen and progesterone receptors in the trophoblast .
	manualset3
142141	3	408843	5	NULL	NULL	NULL	NULL	estrogen receptors 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The author demonstrates the presence of estrogen and progesterone receptors in the trophoblast .
	manualset3
142142	4	408843	5	NULL	NULL	0	NULL	progesterone receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The author demonstrates the presence of estrogen and progesterone receptors in the trophoblast .
	manualset3
142143	5	408843	5	NULL	NULL	0	NULL	trophoblast 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The author demonstrates the presence of estrogen and progesterone receptors in the trophoblast .
	manualset3
142144	1	408844	5	NULL	NULL	0	NULL	screen 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A screen for NAB-regulated genes identified several ( including Id2 , Id4 , and Rad ) that declined during the course of peripheral nerve myelination .
	manualset3
142145	2	408844	5	NULL	NULL	0	NULL	NAB-regulated genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A screen for NAB-regulated genes identified several ( including Id2 , Id4 , and Rad ) that declined during the course of peripheral nerve myelination .
	manualset3
142146	3	408844	5	NULL	NULL	0	NULL	Id2 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A screen for NAB-regulated genes identified several ( including Id2 , Id4 , and Rad ) that declined during the course of peripheral nerve myelination .
	manualset3
142147	4	408844	5	NULL	NULL	0	NULL	Id4 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A screen for NAB-regulated genes identified several ( including Id2 , Id4 , and Rad ) that declined during the course of peripheral nerve myelination .
	manualset3
142148	5	408844	5	NULL	NULL	0	NULL	Rad 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A screen for NAB-regulated genes identified several ( including Id2 , Id4 , and Rad ) that declined during the course of peripheral nerve myelination .
	manualset3
142149	6	408844	5	NULL	NULL	0	NULL	course 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A screen for NAB-regulated genes identified several ( including Id2 , Id4 , and Rad ) that declined during the course of peripheral nerve myelination .
	manualset3
142150	7	408844	5	NULL	NULL	0	NULL	peripheral nerve myelination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A screen for NAB-regulated genes identified several ( including Id2 , Id4 , and Rad ) that declined during the course of peripheral nerve myelination .
	manualset3
142151	1	408845	5	NULL	NULL	0	NULL	author 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The author discusses this measurement process that allows managers to evaluate where they are and where they want to be , and to set a course of action that closes the gap between the two .
	manualset3
142152	2	408845	5	NULL	NULL	0	NULL	measurement process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The author discusses this measurement process that allows managers to evaluate where they are and where they want to be , and to set a course of action that closes the gap between the two .
	manualset3
142153	3	408845	5	NULL	NULL	0	NULL	managers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The author discusses this measurement process that allows managers to evaluate where they are and where they want to be , and to set a course of action that closes the gap between the two .
	manualset3
142154	4	408845	5	NULL	NULL	0	NULL	course of action	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The author discusses this measurement process that allows managers to evaluate where they are and where they want to be , and to set a course of action that closes the gap between the two .
	manualset3
142155	5	408845	5	NULL	NULL	0	NULL	gap 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The author discusses this measurement process that allows managers to evaluate where they are and where they want to be , and to set a course of action that closes the gap between the two .
	manualset3
142156	6	408845	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The author discusses this measurement process that allows managers to evaluate where they are and where they want to be , and to set a course of action that closes the gap between the two .
	manualset3
142157	1	408846	5	NULL	NULL	0	NULL	author 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The author explains how Maryland hospitals ' analysis of mortality data has enabled them to explain variations to the public and improve their quality assurance programs .
	manualset3
142158	2	408846	5	NULL	NULL	0	NULL	Maryland hospitals ' analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The author explains how Maryland hospitals ' analysis of mortality data has enabled them to explain variations to the public and improve their quality assurance programs .
	manualset3
142159	3	408846	5	NULL	NULL	0	NULL	mortality data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The author explains how Maryland hospitals ' analysis of mortality data has enabled them to explain variations to the public and improve their quality assurance programs .
	manualset3
142160	4	408846	5	NULL	NULL	0	NULL	variations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The author explains how Maryland hospitals ' analysis of mortality data has enabled them to explain variations to the public and improve their quality assurance programs .
	manualset3
142161	5	408846	5	NULL	NULL	0	NULL	public 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The author explains how Maryland hospitals ' analysis of mortality data has enabled them to explain variations to the public and improve their quality assurance programs .
	manualset3
142162	6	408846	5	NULL	NULL	0	NULL	quality assurance programs	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The author explains how Maryland hospitals ' analysis of mortality data has enabled them to explain variations to the public and improve their quality assurance programs .
	manualset3
142163	1	408847	5	NULL	NULL	0	NULL	author 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The author has extended its application to various parts of the skeleton and presents his experience which extends over more than 15 years .
	manualset3
142164	2	408847	5	NULL	NULL	0	NULL	application 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The author has extended its application to various parts of the skeleton and presents his experience which extends over more than 15 years .
	manualset3
142165	3	408847	5	NULL	NULL	0	NULL	parts of the skeleton	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The author has extended its application to various parts of the skeleton and presents his experience which extends over more than 15 years .
	manualset3
142166	4	408847	5	NULL	NULL	0	NULL	experience 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The author has extended its application to various parts of the skeleton and presents his experience which extends over more than 15 years .
	manualset3
142167	5	408847	5	NULL	NULL	0	NULL	15 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The author has extended its application to various parts of the skeleton and presents his experience which extends over more than 15 years .
	manualset3
142168	1	408848	5	NULL	NULL	0	NULL	author 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The author investigates trends in rural-urban migration in Mexico , using data from the 1990 census .
	manualset3
142169	2	408848	5	NULL	NULL	0	NULL	trends 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The author investigates trends in rural-urban migration in Mexico , using data from the 1990 census .
	manualset3
142170	3	408848	5	NULL	NULL	0	NULL	rural-urban migration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The author investigates trends in rural-urban migration in Mexico , using data from the 1990 census .
	manualset3
142171	4	408848	5	NULL	NULL	0	NULL	Mexico 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The author investigates trends in rural-urban migration in Mexico , using data from the 1990 census .
	manualset3
142172	5	408848	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The author investigates trends in rural-urban migration in Mexico , using data from the 1990 census .
	manualset3
142173	6	408848	5	NULL	NULL	0	NULL	1990 census	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The author investigates trends in rural-urban migration in Mexico , using data from the 1990 census .
	manualset3
142174	1	408849	5	NULL	NULL	0	NULL	author 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The author presents the DIALOGUE system , a method of communication designed to make a smooth transition to ADA compliance in the fieldwork arena .
	manualset3
142175	2	408849	5	NULL	NULL	0	NULL	DIALOGUE system	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The author presents the DIALOGUE system , a method of communication designed to make a smooth transition to ADA compliance in the fieldwork arena .
	manualset3
142176	3	408849	5	NULL	NULL	0	NULL	method of communication	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The author presents the DIALOGUE system , a method of communication designed to make a smooth transition to ADA compliance in the fieldwork arena .
	manualset3
142177	4	408849	5	NULL	NULL	0	NULL	smooth transition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The author presents the DIALOGUE system , a method of communication designed to make a smooth transition to ADA compliance in the fieldwork arena .
	manualset3
142178	5	408849	5	NULL	NULL	0	NULL	ADA compliance	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The author presents the DIALOGUE system , a method of communication designed to make a smooth transition to ADA compliance in the fieldwork arena .
	manualset3
142179	6	408849	5	NULL	NULL	0	NULL	fieldwork arena	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The author presents the DIALOGUE system , a method of communication designed to make a smooth transition to ADA compliance in the fieldwork arena .
	manualset3
142180	1	408850	5	NULL	NULL	0	NULL	author 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The author provides a detailed analysis of the present economic and social situation of the elderly in Romania .
	manualset3
142181	2	408850	5	NULL	NULL	0	NULL	analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The author provides a detailed analysis of the present economic and social situation of the elderly in Romania .
	manualset3
142182	3	408850	5	NULL	NULL	0	NULL	economic situation 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The author provides a detailed analysis of the present economic and social situation of the elderly in Romania .
	manualset3
142183	4	408850	5	NULL	NULL	0	NULL	social situation 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The author provides a detailed analysis of the present economic and social situation of the elderly in Romania .
	manualset3
142184	5	408850	5	NULL	NULL	0	NULL	elderly 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The author provides a detailed analysis of the present economic and social situation of the elderly in Romania .
	manualset3
142185	6	408850	5	NULL	NULL	0	NULL	Romania 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The author provides a detailed analysis of the present economic and social situation of the elderly in Romania .
	manualset3
142186	1	408851	5	NULL	NULL	0	NULL	author 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The author recommends routine dissection of all 4 parathyroids , and removal of the one or possibly two large glands when the others perfectly identified are normal .
	manualset3
142187	2	408851	5	NULL	NULL	NULL	NULL	routine dissection 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The author recommends routine dissection of all 4 parathyroids , and removal of the one or possibly two large glands when the others perfectly identified are normal .
	manualset3
142188	3	408851	5	NULL	NULL	0	NULL	4 parathyroids	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The author recommends routine dissection of all 4 parathyroids , and removal of the one or possibly two large glands when the others perfectly identified are normal .
	manualset3
142189	4	408851	5	NULL	NULL	0	NULL	removal 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The author recommends routine dissection of all 4 parathyroids , and removal of the one or possibly two large glands when the others perfectly identified are normal .
	manualset3
142190	5	408851	5	NULL	NULL	0	NULL	one 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The author recommends routine dissection of all 4 parathyroids , and removal of the one or possibly two large glands when the others perfectly identified are normal .
	manualset3
142191	6	408851	5	NULL	NULL	0	NULL	two large glands 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The author recommends routine dissection of all 4 parathyroids , and removal of the one or possibly two large glands when the others perfectly identified are normal .
	manualset3
142192	1	408852	5	NULL	NULL	0	NULL	author 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The author reports a case of Nora 's lesion of the proximal phalanx of the second toe , successfully managed by en bloc excision of the swelling .
	manualset3
142193	2	408852	5	NULL	NULL	0	NULL	case 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The author reports a case of Nora 's lesion of the proximal phalanx of the second toe , successfully managed by en bloc excision of the swelling .
	manualset3
142194	3	408852	5	NULL	NULL	0	NULL	Nora 's lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The author reports a case of Nora 's lesion of the proximal phalanx of the second toe , successfully managed by en bloc excision of the swelling .
	manualset3
142195	4	408852	5	NULL	NULL	0	NULL	proximal phalanx 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The author reports a case of Nora 's lesion of the proximal phalanx of the second toe , successfully managed by en bloc excision of the swelling .
	manualset3
142196	5	408852	5	NULL	NULL	0	NULL	second toe	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The author reports a case of Nora 's lesion of the proximal phalanx of the second toe , successfully managed by en bloc excision of the swelling .
	manualset3
142197	6	408852	5	NULL	NULL	0	NULL	en bloc excision 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The author reports a case of Nora 's lesion of the proximal phalanx of the second toe , successfully managed by en bloc excision of the swelling .
	manualset3
142198	7	408852	5	NULL	NULL	0	NULL	swelling 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The author reports a case of Nora 's lesion of the proximal phalanx of the second toe , successfully managed by en bloc excision of the swelling .
	manualset3
142199	1	408853	5	NULL	NULL	0	NULL	author 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The author reviewed the case records of 100 physician inpatients in a private psychiatric hospital .
	manualset3
142200	2	408853	5	NULL	NULL	0	NULL	case records	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The author reviewed the case records of 100 physician inpatients in a private psychiatric hospital .
	manualset3
142201	3	408853	5	NULL	NULL	0	NULL	100 physician inpatients	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The author reviewed the case records of 100 physician inpatients in a private psychiatric hospital .
	manualset3
142202	4	408853	5	NULL	NULL	0	NULL	private psychiatric hospital 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The author reviewed the case records of 100 physician inpatients in a private psychiatric hospital .
	manualset3
142203	1	408854	5	NULL	NULL	0	NULL	seasonal variability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A seasonal variability of trace metal concentrations and antioxidant enzymes was observed in gills and digestive gland of the Mediterranean mussel Mytilus galloprovincialis from both a polluted and a nonpolluted population .
	manualset3
142204	2	408854	5	NULL	NULL	0	NULL	trace metal concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A seasonal variability of trace metal concentrations and antioxidant enzymes was observed in gills and digestive gland of the Mediterranean mussel Mytilus galloprovincialis from both a polluted and a nonpolluted population .
	manualset3
142205	3	408854	5	NULL	NULL	0	NULL	antioxidant enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A seasonal variability of trace metal concentrations and antioxidant enzymes was observed in gills and digestive gland of the Mediterranean mussel Mytilus galloprovincialis from both a polluted and a nonpolluted population .
	manualset3
142206	4	408854	5	NULL	NULL	0	NULL	gills 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A seasonal variability of trace metal concentrations and antioxidant enzymes was observed in gills and digestive gland of the Mediterranean mussel Mytilus galloprovincialis from both a polluted and a nonpolluted population .
	manualset3
142207	5	408854	5	NULL	NULL	0	NULL	digestive gland	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A seasonal variability of trace metal concentrations and antioxidant enzymes was observed in gills and digestive gland of the Mediterranean mussel Mytilus galloprovincialis from both a polluted and a nonpolluted population .
	manualset3
142208	6	408854	5	NULL	NULL	0	NULL	Mediterranean mussel Mytilus galloprovincialis 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A seasonal variability of trace metal concentrations and antioxidant enzymes was observed in gills and digestive gland of the Mediterranean mussel Mytilus galloprovincialis from both a polluted and a nonpolluted population .
	manualset3
142209	7	408854	5	NULL	NULL	0	NULL	polluted population 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A seasonal variability of trace metal concentrations and antioxidant enzymes was observed in gills and digestive gland of the Mediterranean mussel Mytilus galloprovincialis from both a polluted and a nonpolluted population .
	manualset3
142210	8	408854	5	NULL	NULL	0	NULL	nonpolluted population 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A seasonal variability of trace metal concentrations and antioxidant enzymes was observed in gills and digestive gland of the Mediterranean mussel Mytilus galloprovincialis from both a polluted and a nonpolluted population .
	manualset3
142211	1	408855	5	NULL	NULL	0	NULL	authors ' data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors ' data suggest that p53 mutation may play an important role in the pathogenesis of lung cancer of silicotic patients .
	manualset3
142212	2	408855	5	NULL	NULL	0	NULL	 p53 mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors ' data suggest that p53 mutation may play an important role in the pathogenesis of lung cancer of silicotic patients .
	manualset3
142213	3	408855	5	NULL	NULL	0	NULL	important role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors ' data suggest that p53 mutation may play an important role in the pathogenesis of lung cancer of silicotic patients .
	manualset3
142214	4	408855	5	NULL	NULL	0	NULL	pathogenesis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors ' data suggest that p53 mutation may play an important role in the pathogenesis of lung cancer of silicotic patients .
	manualset3
142215	5	408855	5	NULL	NULL	0	NULL	lung cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors ' data suggest that p53 mutation may play an important role in the pathogenesis of lung cancer of silicotic patients .
	manualset3
142216	6	408855	5	NULL	NULL	0	NULL	silicotic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors ' data suggest that p53 mutation may play an important role in the pathogenesis of lung cancer of silicotic patients .
	manualset3
142217	1	408856	5	NULL	NULL	0	NULL	authors ' findings	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors ' findings indicate that only approximately 5 % of the cortical signal in ( + ) - ( 11C ) DTBZ scans results from binding to VMAT2 sites .
	manualset3
142218	2	408856	5	NULL	NULL	0	NULL	5 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors ' findings indicate that only approximately 5 % of the cortical signal in ( + ) - ( 11C ) DTBZ scans results from binding to VMAT2 sites .
	manualset3
142219	3	408856	5	NULL	NULL	0	NULL	cortical signal	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors ' findings indicate that only approximately 5 % of the cortical signal in ( + ) - ( 11C ) DTBZ scans results from binding to VMAT2 sites .
	manualset3
142220	4	408856	5	NULL	NULL	NULL	NULL	 ( + ) - ( 11C ) DTBZ scans results 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The authors ' findings indicate that only approximately 5 % of the cortical signal in ( + ) - ( 11C ) DTBZ scans results from binding to VMAT2 sites .
	manualset3
142221	5	408856	5	NULL	NULL	0	NULL	VMAT2 sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors ' findings indicate that only approximately 5 % of the cortical signal in ( + ) - ( 11C ) DTBZ scans results from binding to VMAT2 sites .
	manualset3
142222	1	408857	5	NULL	NULL	0	NULL	animal model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors ' search for an animal model of amnesia , based on ablations aimed at the hippocampal formation in infant rhesus monkeys , provides support for this view .
	manualset3
142223	2	408857	5	NULL	NULL	0	NULL	amnesia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors ' search for an animal model of amnesia , based on ablations aimed at the hippocampal formation in infant rhesus monkeys , provides support for this view .
	manualset3
142224	3	408857	5	NULL	NULL	0	NULL	ablations 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors ' search for an animal model of amnesia , based on ablations aimed at the hippocampal formation in infant rhesus monkeys , provides support for this view .
	manualset3
142225	4	408857	5	NULL	NULL	0	NULL	hippocampal formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors ' search for an animal model of amnesia , based on ablations aimed at the hippocampal formation in infant rhesus monkeys , provides support for this view .
	manualset3
142226	5	408857	5	NULL	NULL	0	NULL	infant rhesus monkeys 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors ' search for an animal model of amnesia , based on ablations aimed at the hippocampal formation in infant rhesus monkeys , provides support for this view .
	manualset3
142227	6	408857	5	NULL	NULL	0	NULL	view 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors ' search for an animal model of amnesia , based on ablations aimed at the hippocampal formation in infant rhesus monkeys , provides support for this view .
	manualset3
142228	1	408858	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors also mention the laboratory methods that are currently being used to classify more precisely the vasculitides associated with glomerulonephritis .
	manualset3
142229	2	408858	5	NULL	NULL	0	NULL	laboratory methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors also mention the laboratory methods that are currently being used to classify more precisely the vasculitides associated with glomerulonephritis .
	manualset3
142230	3	408858	5	NULL	NULL	0	NULL	vasculitides 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors also mention the laboratory methods that are currently being used to classify more precisely the vasculitides associated with glomerulonephritis .
	manualset3
142231	4	408858	5	NULL	NULL	0	NULL	glomerulonephritis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors also mention the laboratory methods that are currently being used to classify more precisely the vasculitides associated with glomerulonephritis .
	manualset3
142232	1	408859	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors also refer to recent data on the most frequently identified antibiotic resistance of respiratory pathogens .
	manualset3
142233	2	408859	5	NULL	NULL	0	NULL	recent data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors also refer to recent data on the most frequently identified antibiotic resistance of respiratory pathogens .
	manualset3
142234	3	408859	5	NULL	NULL	0	NULL	antibiotic resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors also refer to recent data on the most frequently identified antibiotic resistance of respiratory pathogens .
	manualset3
142235	4	408859	5	NULL	NULL	0	NULL	respiratory pathogens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors also refer to recent data on the most frequently identified antibiotic resistance of respiratory pathogens .
	manualset3
142236	1	408860	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors analyze a group of 27 patients with carcinoma of the rectum who were treated in the authors ' department in 1975-1990 by electrocoagulation .
	manualset3
142237	2	408860	5	NULL	NULL	0	NULL	group of 27 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors analyze a group of 27 patients with carcinoma of the rectum who were treated in the authors ' department in 1975-1990 by electrocoagulation .
	manualset3
142238	3	408860	5	NULL	NULL	0	NULL	carcinoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors analyze a group of 27 patients with carcinoma of the rectum who were treated in the authors ' department in 1975-1990 by electrocoagulation .
	manualset3
142239	4	408860	5	NULL	NULL	0	NULL	rectum 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors analyze a group of 27 patients with carcinoma of the rectum who were treated in the authors ' department in 1975-1990 by electrocoagulation .
	manualset3
142240	5	408860	5	NULL	NULL	0	NULL	authors ' department	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors analyze a group of 27 patients with carcinoma of the rectum who were treated in the authors ' department in 1975-1990 by electrocoagulation .
	manualset3
142241	6	408860	5	NULL	NULL	0	NULL	1975-1990 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors analyze a group of 27 patients with carcinoma of the rectum who were treated in the authors ' department in 1975-1990 by electrocoagulation .
	manualset3
142242	7	408860	5	NULL	NULL	0	NULL	electrocoagulation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors analyze a group of 27 patients with carcinoma of the rectum who were treated in the authors ' department in 1975-1990 by electrocoagulation .
	manualset3
142243	1	408861	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors analyze the structural properties and robustness of a discussion network about mercury issues in a community in the Brazilian Amazon involved in a participatory research aimed at reducing exposure to the pollutant .
	manualset3
142244	2	408861	5	NULL	NULL	0	NULL	structural properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors analyze the structural properties and robustness of a discussion network about mercury issues in a community in the Brazilian Amazon involved in a participatory research aimed at reducing exposure to the pollutant .
	manualset3
142245	3	408861	5	NULL	NULL	0	NULL	robustness 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors analyze the structural properties and robustness of a discussion network about mercury issues in a community in the Brazilian Amazon involved in a participatory research aimed at reducing exposure to the pollutant .
	manualset3
142246	4	408861	5	NULL	NULL	0	NULL	discussion network 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors analyze the structural properties and robustness of a discussion network about mercury issues in a community in the Brazilian Amazon involved in a participatory research aimed at reducing exposure to the pollutant .
	manualset3
142247	5	408861	5	NULL	NULL	0	NULL	mercury issues	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors analyze the structural properties and robustness of a discussion network about mercury issues in a community in the Brazilian Amazon involved in a participatory research aimed at reducing exposure to the pollutant .
	manualset3
142248	6	408861	5	NULL	NULL	0	NULL	community 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors analyze the structural properties and robustness of a discussion network about mercury issues in a community in the Brazilian Amazon involved in a participatory research aimed at reducing exposure to the pollutant .
	manualset3
142249	7	408861	5	NULL	NULL	0	NULL	Brazilian Amazon	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors analyze the structural properties and robustness of a discussion network about mercury issues in a community in the Brazilian Amazon involved in a participatory research aimed at reducing exposure to the pollutant .
	manualset3
142250	8	408861	5	NULL	NULL	0	NULL	participatory research 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors analyze the structural properties and robustness of a discussion network about mercury issues in a community in the Brazilian Amazon involved in a participatory research aimed at reducing exposure to the pollutant .
	manualset3
142251	9	408861	5	NULL	NULL	0	NULL	exposure 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors analyze the structural properties and robustness of a discussion network about mercury issues in a community in the Brazilian Amazon involved in a participatory research aimed at reducing exposure to the pollutant .
	manualset3
142252	10	408861	5	NULL	NULL	0	NULL	pollutant 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors analyze the structural properties and robustness of a discussion network about mercury issues in a community in the Brazilian Amazon involved in a participatory research aimed at reducing exposure to the pollutant .
	manualset3
142253	1	408862	5	NULL	NULL	NULL	NULL	second episode	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A second episode of ganglion cell death takes place when an optic nerve regenerates for a second time in the frog .
	manualset3
142254	2	408862	5	NULL	NULL	0	NULL	ganglion cell death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A second episode of ganglion cell death takes place when an optic nerve regenerates for a second time in the frog .
	manualset3
142255	3	408862	5	NULL	NULL	0	NULL	optic nerve	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A second episode of ganglion cell death takes place when an optic nerve regenerates for a second time in the frog .
	manualset3
142256	4	408862	5	NULL	NULL	0	NULL	second time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	A second episode of ganglion cell death takes place when an optic nerve regenerates for a second time in the frog .
	manualset3
142257	5	408862	5	NULL	NULL	0	NULL	frog 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A second episode of ganglion cell death takes place when an optic nerve regenerates for a second time in the frog .
	manualset3
142258	1	408863	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors analyzed 133 boy cases and 399 sex-matched controls extracted from a population-based study of NNT conducted in Punjab Province , Pakistan .
	manualset3
142259	2	408863	5	NULL	NULL	0	NULL	133 boy cases	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors analyzed 133 boy cases and 399 sex-matched controls extracted from a population-based study of NNT conducted in Punjab Province , Pakistan .
	manualset3
142260	3	408863	5	NULL	NULL	0	NULL	399 sex-matched controls	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors analyzed 133 boy cases and 399 sex-matched controls extracted from a population-based study of NNT conducted in Punjab Province , Pakistan .
	manualset3
142261	4	408863	5	NULL	NULL	0	NULL	population-based study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors analyzed 133 boy cases and 399 sex-matched controls extracted from a population-based study of NNT conducted in Punjab Province , Pakistan .
	manualset3
142262	5	408863	5	NULL	NULL	0	NULL	NNT 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors analyzed 133 boy cases and 399 sex-matched controls extracted from a population-based study of NNT conducted in Punjab Province , Pakistan .
	manualset3
142263	6	408863	5	NULL	NULL	0	NULL	Punjab Province , Pakistan	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors analyzed 133 boy cases and 399 sex-matched controls extracted from a population-based study of NNT conducted in Punjab Province , Pakistan .
	manualset3
142264	1	408864	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors are presenting seven patients who had operations between July 1984 and July 1985 and who developed herpes infections postoperatively .
	manualset3
142265	2	408864	5	NULL	NULL	0	NULL	seven patients 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors are presenting seven patients who had operations between July 1984 and July 1985 and who developed herpes infections postoperatively .
	manualset3
142266	3	408864	5	NULL	NULL	0	NULL	operations 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors are presenting seven patients who had operations between July 1984 and July 1985 and who developed herpes infections postoperatively .
	manualset3
142267	4	408864	5	NULL	NULL	0	NULL	between July 1984 and July 1985 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors are presenting seven patients who had operations between July 1984 and July 1985 and who developed herpes infections postoperatively .
	manualset3
142268	5	408864	5	NULL	NULL	0	NULL	herpes infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors are presenting seven patients who had operations between July 1984 and July 1985 and who developed herpes infections postoperatively .
	manualset3
142269	1	408865	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors assess the equivalence of 2 assays and put forward a general approach for assay agreement analysis that can be applied during drug discovery .
	manualset3
142270	2	408865	5	NULL	NULL	0	NULL	equivalence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors assess the equivalence of 2 assays and put forward a general approach for assay agreement analysis that can be applied during drug discovery .
	manualset3
142271	3	408865	5	NULL	NULL	0	NULL	2 assays 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors assess the equivalence of 2 assays and put forward a general approach for assay agreement analysis that can be applied during drug discovery .
	manualset3
142272	4	408865	5	NULL	NULL	0	NULL	general approach	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors assess the equivalence of 2 assays and put forward a general approach for assay agreement analysis that can be applied during drug discovery .
	manualset3
142273	5	408865	5	NULL	NULL	0	NULL	assay agreement analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors assess the equivalence of 2 assays and put forward a general approach for assay agreement analysis that can be applied during drug discovery .
	manualset3
142274	6	408865	5	NULL	NULL	0	NULL	drug discovery	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors assess the equivalence of 2 assays and put forward a general approach for assay agreement analysis that can be applied during drug discovery .
	manualset3
142275	1	408866	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors assessed the outcome of surgery for this lesion in relation to causative factors and diagnostic imaging ( computerized tomography ( CT ) , CT myelography ) , as well as eventual preservation of the subarachnoid space .
	manualset3
142276	2	408866	5	NULL	NULL	0	NULL	outcome 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors assessed the outcome of surgery for this lesion in relation to causative factors and diagnostic imaging ( computerized tomography ( CT ) , CT myelography ) , as well as eventual preservation of the subarachnoid space .
	manualset3
142277	3	408866	5	NULL	NULL	0	NULL	surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors assessed the outcome of surgery for this lesion in relation to causative factors and diagnostic imaging ( computerized tomography ( CT ) , CT myelography ) , as well as eventual preservation of the subarachnoid space .
	manualset3
142278	4	408866	5	NULL	NULL	0	NULL	lesion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors assessed the outcome of surgery for this lesion in relation to causative factors and diagnostic imaging ( computerized tomography ( CT ) , CT myelography ) , as well as eventual preservation of the subarachnoid space .
	manualset3
142279	5	408866	5	NULL	NULL	0	NULL	causative factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors assessed the outcome of surgery for this lesion in relation to causative factors and diagnostic imaging ( computerized tomography ( CT ) , CT myelography ) , as well as eventual preservation of the subarachnoid space .
	manualset3
142280	6	408866	5	NULL	NULL	0	NULL	diagnostic imaging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors assessed the outcome of surgery for this lesion in relation to causative factors and diagnostic imaging ( computerized tomography ( CT ) , CT myelography ) , as well as eventual preservation of the subarachnoid space .
	manualset3
142281	7	408866	5	NULL	NULL	0	NULL	computerized tomography ( CT )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors assessed the outcome of surgery for this lesion in relation to causative factors and diagnostic imaging ( computerized tomography ( CT ) , CT myelography ) , as well as eventual preservation of the subarachnoid space .
	manualset3
142282	8	408866	5	NULL	NULL	0	NULL	 CT myelography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors assessed the outcome of surgery for this lesion in relation to causative factors and diagnostic imaging ( computerized tomography ( CT ) , CT myelography ) , as well as eventual preservation of the subarachnoid space .
	manualset3
142283	9	408866	5	NULL	NULL	0	NULL	eventual preservation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors assessed the outcome of surgery for this lesion in relation to causative factors and diagnostic imaging ( computerized tomography ( CT ) , CT myelography ) , as well as eventual preservation of the subarachnoid space .
	manualset3
142284	10	408866	5	NULL	NULL	0	NULL	subarachnoid space	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors assessed the outcome of surgery for this lesion in relation to causative factors and diagnostic imaging ( computerized tomography ( CT ) , CT myelography ) , as well as eventual preservation of the subarachnoid space .
	manualset3
142285	1	408867	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors believe that legislation could effectively support the job of prevention and education , which physicians may carry out in order to save little girls from the risk of familial tradition of genital mutilations .
	manualset3
142286	2	408867	5	NULL	NULL	0	NULL	legislation 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors believe that legislation could effectively support the job of prevention and education , which physicians may carry out in order to save little girls from the risk of familial tradition of genital mutilations .
	manualset3
142287	3	408867	5	NULL	NULL	0	NULL	job of prevention and education	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors believe that legislation could effectively support the job of prevention and education , which physicians may carry out in order to save little girls from the risk of familial tradition of genital mutilations .
	manualset3
142288	4	408867	5	NULL	NULL	0	NULL	physicians 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors believe that legislation could effectively support the job of prevention and education , which physicians may carry out in order to save little girls from the risk of familial tradition of genital mutilations .
	manualset3
142289	5	408867	5	NULL	NULL	0	NULL	little girls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors believe that legislation could effectively support the job of prevention and education , which physicians may carry out in order to save little girls from the risk of familial tradition of genital mutilations .
	manualset3
142290	6	408867	5	NULL	NULL	0	NULL	risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors believe that legislation could effectively support the job of prevention and education , which physicians may carry out in order to save little girls from the risk of familial tradition of genital mutilations .
	manualset3
142291	7	408867	5	NULL	NULL	0	NULL	familial tradition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors believe that legislation could effectively support the job of prevention and education , which physicians may carry out in order to save little girls from the risk of familial tradition of genital mutilations .
	manualset3
142292	8	408867	5	NULL	NULL	0	NULL	genital mutilations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors believe that legislation could effectively support the job of prevention and education , which physicians may carry out in order to save little girls from the risk of familial tradition of genital mutilations .
	manualset3
142293	1	408868	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors compared efficacy and safety of risperidone and clozapine for the treatment of psychosis in a double-blind trial with 10 subjects with Parkinson 's disease ( PD ) and psychosis .
	manualset3
142294	2	408868	5	NULL	NULL	0	NULL	efficacy 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors compared efficacy and safety of risperidone and clozapine for the treatment of psychosis in a double-blind trial with 10 subjects with Parkinson 's disease ( PD ) and psychosis .
	manualset3
142295	3	408868	5	NULL	NULL	0	NULL	safety 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors compared efficacy and safety of risperidone and clozapine for the treatment of psychosis in a double-blind trial with 10 subjects with Parkinson 's disease ( PD ) and psychosis .
	manualset3
142296	4	408868	5	NULL	NULL	0	NULL	risperidone 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors compared efficacy and safety of risperidone and clozapine for the treatment of psychosis in a double-blind trial with 10 subjects with Parkinson 's disease ( PD ) and psychosis .
	manualset3
142297	5	408868	5	NULL	NULL	0	NULL	clozapine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors compared efficacy and safety of risperidone and clozapine for the treatment of psychosis in a double-blind trial with 10 subjects with Parkinson 's disease ( PD ) and psychosis .
	manualset3
142298	6	408868	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors compared efficacy and safety of risperidone and clozapine for the treatment of psychosis in a double-blind trial with 10 subjects with Parkinson 's disease ( PD ) and psychosis .
	manualset3
142299	7	408868	5	NULL	NULL	0	NULL	psychosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors compared efficacy and safety of risperidone and clozapine for the treatment of psychosis in a double-blind trial with 10 subjects with Parkinson 's disease ( PD ) and psychosis .
	manualset3
142300	8	408868	5	NULL	NULL	0	NULL	double-blind trial 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors compared efficacy and safety of risperidone and clozapine for the treatment of psychosis in a double-blind trial with 10 subjects with Parkinson 's disease ( PD ) and psychosis .
	manualset3
142301	9	408868	5	NULL	NULL	0	NULL	10 subjects	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors compared efficacy and safety of risperidone and clozapine for the treatment of psychosis in a double-blind trial with 10 subjects with Parkinson 's disease ( PD ) and psychosis .
	manualset3
142302	10	408868	5	NULL	NULL	0	NULL	Parkinson 's disease ( PD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors compared efficacy and safety of risperidone and clozapine for the treatment of psychosis in a double-blind trial with 10 subjects with Parkinson 's disease ( PD ) and psychosis .
	manualset3
142303	11	408868	5	NULL	NULL	0	NULL	psychosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors compared efficacy and safety of risperidone and clozapine for the treatment of psychosis in a double-blind trial with 10 subjects with Parkinson 's disease ( PD ) and psychosis .
	manualset3
142304	1	408869	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors compared marital satisfaction of men and women in the neurotic and the control group .
	manualset3
142305	2	408869	5	NULL	NULL	0	NULL	marital satisfaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors compared marital satisfaction of men and women in the neurotic and the control group .
	manualset3
142306	3	408869	5	NULL	NULL	0	NULL	men 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors compared marital satisfaction of men and women in the neurotic and the control group .
	manualset3
142307	4	408869	5	NULL	NULL	0	NULL	women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors compared marital satisfaction of men and women in the neurotic and the control group .
	manualset3
142308	5	408869	5	NULL	NULL	0	NULL	neurotic  group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors compared marital satisfaction of men and women in the neurotic and the control group .
	manualset3
142309	6	408869	5	NULL	NULL	0	NULL	control group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors compared marital satisfaction of men and women in the neurotic and the control group .
	manualset3
142310	1	408870	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that 99mTc HIDA scanning is a valuable , minimally invasive method of diagnosing papillary stenosis .
	manualset3
142311	2	408870	5	NULL	NULL	0	NULL	99mTc HIDA scanning	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that 99mTc HIDA scanning is a valuable , minimally invasive method of diagnosing papillary stenosis .
	manualset3
142312	3	408870	5	NULL	NULL	0	NULL	minimally invasive method	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that 99mTc HIDA scanning is a valuable , minimally invasive method of diagnosing papillary stenosis .
	manualset3
142313	4	408870	5	NULL	NULL	0	NULL	papillary stenosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that 99mTc HIDA scanning is a valuable , minimally invasive method of diagnosing papillary stenosis .
	manualset3
142314	1	408871	5	NULL	NULL	0	NULL	second family	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A second family showed positive linkage to the same 6p23 region with a maximal NPL score 2.125 ( P = 0.0075 ) and LOD score 1.265 .
	manualset3
142315	2	408871	5	NULL	NULL	0	NULL	positive linkage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A second family showed positive linkage to the same 6p23 region with a maximal NPL score 2.125 ( P = 0.0075 ) and LOD score 1.265 .
	manualset3
142316	3	408871	5	NULL	NULL	NULL	NULL	6p23 region	Chromosome												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A second family showed positive linkage to the same 6p23 region with a maximal NPL score 2.125 ( P = 0.0075 ) and LOD score 1.265 .
	manualset3
142317	4	408871	5	NULL	NULL	0	NULL	maximal NPL score	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A second family showed positive linkage to the same 6p23 region with a maximal NPL score 2.125 ( P = 0.0075 ) and LOD score 1.265 .
	manualset3
142318	5	408871	5	NULL	NULL	0	NULL	2.125 ( P = 0.0075 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A second family showed positive linkage to the same 6p23 region with a maximal NPL score 2.125 ( P = 0.0075 ) and LOD score 1.265 .
	manualset3
142319	6	408871	5	NULL	NULL	0	NULL	LOD score	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A second family showed positive linkage to the same 6p23 region with a maximal NPL score 2.125 ( P = 0.0075 ) and LOD score 1.265 .
	manualset3
142320	7	408871	5	NULL	NULL	0	NULL	1.265	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A second family showed positive linkage to the same 6p23 region with a maximal NPL score 2.125 ( P = 0.0075 ) and LOD score 1.265 .
	manualset3
142321	1	408872	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that the most important predictor of outcome following postinfarction aneurysm surgery is the preoperative hemodynamic status of the left ventricle .
	manualset3
142322	2	408872	5	NULL	NULL	0	NULL	important predictor of outcome	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that the most important predictor of outcome following postinfarction aneurysm surgery is the preoperative hemodynamic status of the left ventricle .
	manualset3
142323	3	408872	5	NULL	NULL	0	NULL	postinfarction aneurysm surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that the most important predictor of outcome following postinfarction aneurysm surgery is the preoperative hemodynamic status of the left ventricle .
	manualset3
142324	4	408872	5	NULL	NULL	0	NULL	preoperative hemodynamic status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that the most important predictor of outcome following postinfarction aneurysm surgery is the preoperative hemodynamic status of the left ventricle .
	manualset3
142325	5	408872	5	NULL	NULL	0	NULL	left ventricle 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that the most important predictor of outcome following postinfarction aneurysm surgery is the preoperative hemodynamic status of the left ventricle .
	manualset3
142326	1	408873	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that the primary causes of each scale are the same and that 1 scale measuring the 6 abortion items would be the most balanced way to analyze abortion attitudes and their underlying reasons .
	manualset3
142327	2	408873	5	NULL	NULL	0	NULL	primary causes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that the primary causes of each scale are the same and that 1 scale measuring the 6 abortion items would be the most balanced way to analyze abortion attitudes and their underlying reasons .
	manualset3
142328	3	408873	5	NULL	NULL	NULL	NULL	scale 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The authors conclude that the primary causes of each scale are the same and that 1 scale measuring the 6 abortion items would be the most balanced way to analyze abortion attitudes and their underlying reasons .
	manualset3
142329	4	408873	5	NULL	NULL	0	NULL	 1 scale	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that the primary causes of each scale are the same and that 1 scale measuring the 6 abortion items would be the most balanced way to analyze abortion attitudes and their underlying reasons .
	manualset3
142330	5	408873	5	NULL	NULL	0	NULL	6 abortion items 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that the primary causes of each scale are the same and that 1 scale measuring the 6 abortion items would be the most balanced way to analyze abortion attitudes and their underlying reasons .
	manualset3
142331	6	408873	5	NULL	NULL	0	NULL	abortion attitudes	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that the primary causes of each scale are the same and that 1 scale measuring the 6 abortion items would be the most balanced way to analyze abortion attitudes and their underlying reasons .
	manualset3
142332	7	408873	5	NULL	NULL	0	NULL	underlying reasons	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that the primary causes of each scale are the same and that 1 scale measuring the 6 abortion items would be the most balanced way to analyze abortion attitudes and their underlying reasons .
	manualset3
142333	1	408874	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that the qualities of Mefoxin ( high resistant wide spectrum antibiotic , covering aerobes and anaerobes ) , make it an ideal antibiotic for perioperative prophylaxis in gynaecologic and oncologic surgery ; the clinical effectiveness of Mefoxin in the treatment of inflammatory diseases of the female pelvis precludes the need for a combined parenteral antibiotic therapy .
	manualset3
142334	2	408874	5	NULL	NULL	0	NULL	qualities 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that the qualities of Mefoxin ( high resistant wide spectrum antibiotic , covering aerobes and anaerobes ) , make it an ideal antibiotic for perioperative prophylaxis in gynaecologic and oncologic surgery ; the clinical effectiveness of Mefoxin in the treatment of inflammatory diseases of the female pelvis precludes the need for a combined parenteral antibiotic therapy .
	manualset3
142335	3	408874	5	NULL	NULL	0	NULL	Mefoxin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that the qualities of Mefoxin ( high resistant wide spectrum antibiotic , covering aerobes and anaerobes ) , make it an ideal antibiotic for perioperative prophylaxis in gynaecologic and oncologic surgery ; the clinical effectiveness of Mefoxin in the treatment of inflammatory diseases of the female pelvis precludes the need for a combined parenteral antibiotic therapy .
	manualset3
142336	4	408874	5	NULL	NULL	0	NULL	high resistant wide spectrum antibiotic	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that the qualities of Mefoxin ( high resistant wide spectrum antibiotic , covering aerobes and anaerobes ) , make it an ideal antibiotic for perioperative prophylaxis in gynaecologic and oncologic surgery ; the clinical effectiveness of Mefoxin in the treatment of inflammatory diseases of the female pelvis precludes the need for a combined parenteral antibiotic therapy .
	manualset3
142337	5	408874	5	NULL	NULL	0	NULL	aerobes 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that the qualities of Mefoxin ( high resistant wide spectrum antibiotic , covering aerobes and anaerobes ) , make it an ideal antibiotic for perioperative prophylaxis in gynaecologic and oncologic surgery ; the clinical effectiveness of Mefoxin in the treatment of inflammatory diseases of the female pelvis precludes the need for a combined parenteral antibiotic therapy .
	manualset3
142338	6	408874	5	NULL	NULL	0	NULL	anaerobes 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that the qualities of Mefoxin ( high resistant wide spectrum antibiotic , covering aerobes and anaerobes ) , make it an ideal antibiotic for perioperative prophylaxis in gynaecologic and oncologic surgery ; the clinical effectiveness of Mefoxin in the treatment of inflammatory diseases of the female pelvis precludes the need for a combined parenteral antibiotic therapy .
	manualset3
142339	7	408874	5	NULL	NULL	0	NULL	ideal antibiotic	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that the qualities of Mefoxin ( high resistant wide spectrum antibiotic , covering aerobes and anaerobes ) , make it an ideal antibiotic for perioperative prophylaxis in gynaecologic and oncologic surgery ; the clinical effectiveness of Mefoxin in the treatment of inflammatory diseases of the female pelvis precludes the need for a combined parenteral antibiotic therapy .
	manualset3
142340	8	408874	5	NULL	NULL	0	NULL	perioperative prophylaxis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that the qualities of Mefoxin ( high resistant wide spectrum antibiotic , covering aerobes and anaerobes ) , make it an ideal antibiotic for perioperative prophylaxis in gynaecologic and oncologic surgery ; the clinical effectiveness of Mefoxin in the treatment of inflammatory diseases of the female pelvis precludes the need for a combined parenteral antibiotic therapy .
	manualset3
142341	9	408874	5	NULL	NULL	0	NULL	gynaecologic surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that the qualities of Mefoxin ( high resistant wide spectrum antibiotic , covering aerobes and anaerobes ) , make it an ideal antibiotic for perioperative prophylaxis in gynaecologic and oncologic surgery ; the clinical effectiveness of Mefoxin in the treatment of inflammatory diseases of the female pelvis precludes the need for a combined parenteral antibiotic therapy .
	manualset3
142342	10	408874	5	NULL	NULL	0	NULL	oncologic surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that the qualities of Mefoxin ( high resistant wide spectrum antibiotic , covering aerobes and anaerobes ) , make it an ideal antibiotic for perioperative prophylaxis in gynaecologic and oncologic surgery ; the clinical effectiveness of Mefoxin in the treatment of inflammatory diseases of the female pelvis precludes the need for a combined parenteral antibiotic therapy .
	manualset3
142343	11	408874	5	NULL	NULL	0	NULL	clinical effectiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that the qualities of Mefoxin ( high resistant wide spectrum antibiotic , covering aerobes and anaerobes ) , make it an ideal antibiotic for perioperative prophylaxis in gynaecologic and oncologic surgery ; the clinical effectiveness of Mefoxin in the treatment of inflammatory diseases of the female pelvis precludes the need for a combined parenteral antibiotic therapy .
	manualset3
142344	12	408874	5	NULL	NULL	0	NULL	Mefoxin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that the qualities of Mefoxin ( high resistant wide spectrum antibiotic , covering aerobes and anaerobes ) , make it an ideal antibiotic for perioperative prophylaxis in gynaecologic and oncologic surgery ; the clinical effectiveness of Mefoxin in the treatment of inflammatory diseases of the female pelvis precludes the need for a combined parenteral antibiotic therapy .
	manualset3
142345	13	408874	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that the qualities of Mefoxin ( high resistant wide spectrum antibiotic , covering aerobes and anaerobes ) , make it an ideal antibiotic for perioperative prophylaxis in gynaecologic and oncologic surgery ; the clinical effectiveness of Mefoxin in the treatment of inflammatory diseases of the female pelvis precludes the need for a combined parenteral antibiotic therapy .
	manualset3
142346	14	408874	5	NULL	NULL	0	NULL	inflammatory diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that the qualities of Mefoxin ( high resistant wide spectrum antibiotic , covering aerobes and anaerobes ) , make it an ideal antibiotic for perioperative prophylaxis in gynaecologic and oncologic surgery ; the clinical effectiveness of Mefoxin in the treatment of inflammatory diseases of the female pelvis precludes the need for a combined parenteral antibiotic therapy .
	manualset3
142347	15	408874	5	NULL	NULL	0	NULL	female pelvis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that the qualities of Mefoxin ( high resistant wide spectrum antibiotic , covering aerobes and anaerobes ) , make it an ideal antibiotic for perioperative prophylaxis in gynaecologic and oncologic surgery ; the clinical effectiveness of Mefoxin in the treatment of inflammatory diseases of the female pelvis precludes the need for a combined parenteral antibiotic therapy .
	manualset3
142348	16	408874	5	NULL	NULL	0	NULL	combined parenteral antibiotic therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conclude that the qualities of Mefoxin ( high resistant wide spectrum antibiotic , covering aerobes and anaerobes ) , make it an ideal antibiotic for perioperative prophylaxis in gynaecologic and oncologic surgery ; the clinical effectiveness of Mefoxin in the treatment of inflammatory diseases of the female pelvis precludes the need for a combined parenteral antibiotic therapy .
	manualset3
142349	1	408875	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors concluded that TMR students can profit from reading instruction .
	manualset3
142350	2	408875	5	NULL	NULL	0	NULL	TMR students	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors concluded that TMR students can profit from reading instruction .
	manualset3
142351	3	408875	5	NULL	NULL	0	NULL	instruction 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors concluded that TMR students can profit from reading instruction .
	manualset3
142352	1	408876	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors concluded that an RCT using double-blinded nutritional supplements and targeting apparently healthy individuals is feasible in an intervention study for cancer prevention in Japan .
	manualset3
142353	2	408876	5	NULL	NULL	0	NULL	RCT 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors concluded that an RCT using double-blinded nutritional supplements and targeting apparently healthy individuals is feasible in an intervention study for cancer prevention in Japan .
	manualset3
142354	3	408876	5	NULL	NULL	0	NULL	double-blinded nutritional supplements	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors concluded that an RCT using double-blinded nutritional supplements and targeting apparently healthy individuals is feasible in an intervention study for cancer prevention in Japan .
	manualset3
142355	4	408876	5	NULL	NULL	0	NULL	healthy individuals 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors concluded that an RCT using double-blinded nutritional supplements and targeting apparently healthy individuals is feasible in an intervention study for cancer prevention in Japan .
	manualset3
142356	5	408876	5	NULL	NULL	0	NULL	intervention study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors concluded that an RCT using double-blinded nutritional supplements and targeting apparently healthy individuals is feasible in an intervention study for cancer prevention in Japan .
	manualset3
142357	6	408876	5	NULL	NULL	0	NULL	cancer prevention 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors concluded that an RCT using double-blinded nutritional supplements and targeting apparently healthy individuals is feasible in an intervention study for cancer prevention in Japan .
	manualset3
142358	7	408876	5	NULL	NULL	0	NULL	Japan 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors concluded that an RCT using double-blinded nutritional supplements and targeting apparently healthy individuals is feasible in an intervention study for cancer prevention in Japan .
	manualset3
142359	1	408877	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors concluded that nonrigid instrumentation can be used to achieve successful bony fusion in patients with degenerative spondylolisthesis , who have a preoperative angle difference less than 10 degrees , with excellent clinical results .
	manualset3
142360	2	408877	5	NULL	NULL	0	NULL	nonrigid instrumentation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors concluded that nonrigid instrumentation can be used to achieve successful bony fusion in patients with degenerative spondylolisthesis , who have a preoperative angle difference less than 10 degrees , with excellent clinical results .
	manualset3
142361	3	408877	5	NULL	NULL	0	NULL	bony fusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors concluded that nonrigid instrumentation can be used to achieve successful bony fusion in patients with degenerative spondylolisthesis , who have a preoperative angle difference less than 10 degrees , with excellent clinical results .
	manualset3
142362	4	408877	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors concluded that nonrigid instrumentation can be used to achieve successful bony fusion in patients with degenerative spondylolisthesis , who have a preoperative angle difference less than 10 degrees , with excellent clinical results .
	manualset3
142363	5	408877	5	NULL	NULL	0	NULL	degenerative spondylolisthesis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors concluded that nonrigid instrumentation can be used to achieve successful bony fusion in patients with degenerative spondylolisthesis , who have a preoperative angle difference less than 10 degrees , with excellent clinical results .
	manualset3
142364	6	408877	5	NULL	NULL	0	NULL	preoperative angle difference	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors concluded that nonrigid instrumentation can be used to achieve successful bony fusion in patients with degenerative spondylolisthesis , who have a preoperative angle difference less than 10 degrees , with excellent clinical results .
	manualset3
142365	7	408877	5	NULL	NULL	0	NULL	less than 10 degrees	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors concluded that nonrigid instrumentation can be used to achieve successful bony fusion in patients with degenerative spondylolisthesis , who have a preoperative angle difference less than 10 degrees , with excellent clinical results .
	manualset3
142366	8	408877	5	NULL	NULL	0	NULL	clinical results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors concluded that nonrigid instrumentation can be used to achieve successful bony fusion in patients with degenerative spondylolisthesis , who have a preoperative angle difference less than 10 degrees , with excellent clinical results .
	manualset3
142367	1	408878	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conducted a study using cDNA microarray analysis to determine whether expression levels of genes in tumors were correlated with the outcome of chemotherapy .
	manualset3
142368	2	408878	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conducted a study using cDNA microarray analysis to determine whether expression levels of genes in tumors were correlated with the outcome of chemotherapy .
	manualset3
142369	3	408878	5	NULL	NULL	0	NULL	cDNA microarray analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conducted a study using cDNA microarray analysis to determine whether expression levels of genes in tumors were correlated with the outcome of chemotherapy .
	manualset3
142370	4	408878	5	NULL	NULL	0	NULL	expression levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conducted a study using cDNA microarray analysis to determine whether expression levels of genes in tumors were correlated with the outcome of chemotherapy .
	manualset3
142371	5	408878	5	NULL	NULL	0	NULL	genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conducted a study using cDNA microarray analysis to determine whether expression levels of genes in tumors were correlated with the outcome of chemotherapy .
	manualset3
142372	6	408878	5	NULL	NULL	0	NULL	tumors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conducted a study using cDNA microarray analysis to determine whether expression levels of genes in tumors were correlated with the outcome of chemotherapy .
	manualset3
142373	7	408878	5	NULL	NULL	0	NULL	outcome 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conducted a study using cDNA microarray analysis to determine whether expression levels of genes in tumors were correlated with the outcome of chemotherapy .
	manualset3
142374	8	408878	5	NULL	NULL	0	NULL	chemotherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors conducted a study using cDNA microarray analysis to determine whether expression levels of genes in tumors were correlated with the outcome of chemotherapy .
	manualset3
142375	1	408879	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors describe the case of a patient with right retrocommissural lesion treated by iridiumtherapy and an enormous orostoma which appeared three years later .
	manualset3
142376	2	408879	5	NULL	NULL	NULL	NULL	case 	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The authors describe the case of a patient with right retrocommissural lesion treated by iridiumtherapy and an enormous orostoma which appeared three years later .
	manualset3
142377	3	408879	5	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors describe the case of a patient with right retrocommissural lesion treated by iridiumtherapy and an enormous orostoma which appeared three years later .
	manualset3
142378	4	408879	5	NULL	NULL	0	NULL	right retrocommissural lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors describe the case of a patient with right retrocommissural lesion treated by iridiumtherapy and an enormous orostoma which appeared three years later .
	manualset3
142379	5	408879	5	NULL	NULL	0	NULL	iridiumtherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors describe the case of a patient with right retrocommissural lesion treated by iridiumtherapy and an enormous orostoma which appeared three years later .
	manualset3
142380	6	408879	5	NULL	NULL	0	NULL	enormous orostoma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors describe the case of a patient with right retrocommissural lesion treated by iridiumtherapy and an enormous orostoma which appeared three years later .
	manualset3
142381	7	408879	5	NULL	NULL	0	NULL	three years 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors describe the case of a patient with right retrocommissural lesion treated by iridiumtherapy and an enormous orostoma which appeared three years later .
	manualset3
142382	1	408880	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors describe the focus group process , major findings , and the use of focus group results in a highly multicultural community .
	manualset3
142383	2	408880	5	NULL	NULL	0	NULL	focus group process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors describe the focus group process , major findings , and the use of focus group results in a highly multicultural community .
	manualset3
142384	3	408880	5	NULL	NULL	0	NULL	major findings	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors describe the focus group process , major findings , and the use of focus group results in a highly multicultural community .
	manualset3
142385	4	408880	5	NULL	NULL	0	NULL	use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors describe the focus group process , major findings , and the use of focus group results in a highly multicultural community .
	manualset3
142386	5	408880	5	NULL	NULL	0	NULL	focus group 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors describe the focus group process , major findings , and the use of focus group results in a highly multicultural community .
	manualset3
142387	6	408880	5	NULL	NULL	0	NULL	highly multicultural community 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors describe the focus group process , major findings , and the use of focus group results in a highly multicultural community .
	manualset3
142388	1	408881	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors describe the rural variations and the implications for nurse administrators who often assume an active role in planning and organizing bioethics committees .
	manualset3
142389	2	408881	5	NULL	NULL	0	NULL	rural variations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors describe the rural variations and the implications for nurse administrators who often assume an active role in planning and organizing bioethics committees .
	manualset3
142390	3	408881	5	NULL	NULL	0	NULL	implications 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors describe the rural variations and the implications for nurse administrators who often assume an active role in planning and organizing bioethics committees .
	manualset3
142391	4	408881	5	NULL	NULL	0	NULL	nurse administrators	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors describe the rural variations and the implications for nurse administrators who often assume an active role in planning and organizing bioethics committees .
	manualset3
142392	5	408881	5	NULL	NULL	0	NULL	active role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors describe the rural variations and the implications for nurse administrators who often assume an active role in planning and organizing bioethics committees .
	manualset3
142393	6	408881	5	NULL	NULL	NULL	NULL	bioethics committees	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The authors describe the rural variations and the implications for nurse administrators who often assume an active role in planning and organizing bioethics committees .
	manualset3
142394	1	408882	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors discuss some properties of recent cephalosporin antibiotics and the antibiotics effectiveness in particular of more recent generations of cephalosporins .
	manualset3
142395	2	408882	5	NULL	NULL	0	NULL	properties 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors discuss some properties of recent cephalosporin antibiotics and the antibiotics effectiveness in particular of more recent generations of cephalosporins .
	manualset3
142396	3	408882	5	NULL	NULL	0	NULL	cephalosporin antibiotics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors discuss some properties of recent cephalosporin antibiotics and the antibiotics effectiveness in particular of more recent generations of cephalosporins .
	manualset3
142397	4	408882	5	NULL	NULL	0	NULL	antibiotics effectiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors discuss some properties of recent cephalosporin antibiotics and the antibiotics effectiveness in particular of more recent generations of cephalosporins .
	manualset3
142398	5	408882	5	NULL	NULL	0	NULL	generations 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors discuss some properties of recent cephalosporin antibiotics and the antibiotics effectiveness in particular of more recent generations of cephalosporins .
	manualset3
142399	6	408882	5	NULL	NULL	0	NULL	cephalosporins 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors discuss some properties of recent cephalosporin antibiotics and the antibiotics effectiveness in particular of more recent generations of cephalosporins .
	manualset3
142400	1	408883	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors discuss the role of drug toxicity in the pathogenesis of collagenous enterocolitis .
	manualset3
142401	2	408883	5	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors discuss the role of drug toxicity in the pathogenesis of collagenous enterocolitis .
	manualset3
142402	3	408883	5	NULL	NULL	0	NULL	drug toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors discuss the role of drug toxicity in the pathogenesis of collagenous enterocolitis .
	manualset3
142403	4	408883	5	NULL	NULL	0	NULL	pathogenesis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors discuss the role of drug toxicity in the pathogenesis of collagenous enterocolitis .
	manualset3
142404	5	408883	5	NULL	NULL	0	NULL	collagenous enterocolitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors discuss the role of drug toxicity in the pathogenesis of collagenous enterocolitis .
	manualset3
142405	1	408884	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors draw on social support theory to examine supervisor support match ( support wanted and received ) , support mismatch ( support not wanted and received ) and work outcomes for abused low-wage working women , and to determine if supervisor support match and mismatch are more strongly associated with work outcomes than global supervisor support Face-to-face interviews were conducted with a community sample of abused , employed women who have experienced intimate partner violence ( IPV ) in the past year ( N = 163 ) .
	manualset3
142406	2	408884	5	NULL	NULL	0	NULL	social support theory 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors draw on social support theory to examine supervisor support match ( support wanted and received ) , support mismatch ( support not wanted and received ) and work outcomes for abused low-wage working women , and to determine if supervisor support match and mismatch are more strongly associated with work outcomes than global supervisor support Face-to-face interviews were conducted with a community sample of abused , employed women who have experienced intimate partner violence ( IPV ) in the past year ( N = 163 ) .
	manualset3
142407	3	408884	5	NULL	NULL	NULL	NULL	supervisor support match	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The authors draw on social support theory to examine supervisor support match ( support wanted and received ) , support mismatch ( support not wanted and received ) and work outcomes for abused low-wage working women , and to determine if supervisor support match and mismatch are more strongly associated with work outcomes than global supervisor support Face-to-face interviews were conducted with a community sample of abused , employed women who have experienced intimate partner violence ( IPV ) in the past year ( N = 163 ) .
	manualset3
142408	4	408884	5	NULL	NULL	0	NULL	support mismatch	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors draw on social support theory to examine supervisor support match ( support wanted and received ) , support mismatch ( support not wanted and received ) and work outcomes for abused low-wage working women , and to determine if supervisor support match and mismatch are more strongly associated with work outcomes than global supervisor support Face-to-face interviews were conducted with a community sample of abused , employed women who have experienced intimate partner violence ( IPV ) in the past year ( N = 163 ) .
	manualset3
142409	5	408884	5	NULL	NULL	0	NULL	work outcomes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors draw on social support theory to examine supervisor support match ( support wanted and received ) , support mismatch ( support not wanted and received ) and work outcomes for abused low-wage working women , and to determine if supervisor support match and mismatch are more strongly associated with work outcomes than global supervisor support Face-to-face interviews were conducted with a community sample of abused , employed women who have experienced intimate partner violence ( IPV ) in the past year ( N = 163 ) .
	manualset3
142410	6	408884	5	NULL	NULL	0	NULL	abused low-wage working women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors draw on social support theory to examine supervisor support match ( support wanted and received ) , support mismatch ( support not wanted and received ) and work outcomes for abused low-wage working women , and to determine if supervisor support match and mismatch are more strongly associated with work outcomes than global supervisor support Face-to-face interviews were conducted with a community sample of abused , employed women who have experienced intimate partner violence ( IPV ) in the past year ( N = 163 ) .
	manualset3
142411	7	408884	5	NULL	NULL	0	NULL	supervisor support match	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors draw on social support theory to examine supervisor support match ( support wanted and received ) , support mismatch ( support not wanted and received ) and work outcomes for abused low-wage working women , and to determine if supervisor support match and mismatch are more strongly associated with work outcomes than global supervisor support Face-to-face interviews were conducted with a community sample of abused , employed women who have experienced intimate partner violence ( IPV ) in the past year ( N = 163 ) .
	manualset3
142412	8	408884	5	NULL	NULL	0	NULL	supervisor support mismatch	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors draw on social support theory to examine supervisor support match ( support wanted and received ) , support mismatch ( support not wanted and received ) and work outcomes for abused low-wage working women , and to determine if supervisor support match and mismatch are more strongly associated with work outcomes than global supervisor support Face-to-face interviews were conducted with a community sample of abused , employed women who have experienced intimate partner violence ( IPV ) in the past year ( N = 163 ) .
	manualset3
142413	9	408884	5	NULL	NULL	0	NULL	work outcomes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors draw on social support theory to examine supervisor support match ( support wanted and received ) , support mismatch ( support not wanted and received ) and work outcomes for abused low-wage working women , and to determine if supervisor support match and mismatch are more strongly associated with work outcomes than global supervisor support Face-to-face interviews were conducted with a community sample of abused , employed women who have experienced intimate partner violence ( IPV ) in the past year ( N = 163 ) .
	manualset3
142414	10	408884	5	NULL	NULL	0	NULL	global supervisor support	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors draw on social support theory to examine supervisor support match ( support wanted and received ) , support mismatch ( support not wanted and received ) and work outcomes for abused low-wage working women , and to determine if supervisor support match and mismatch are more strongly associated with work outcomes than global supervisor support Face-to-face interviews were conducted with a community sample of abused , employed women who have experienced intimate partner violence ( IPV ) in the past year ( N = 163 ) .
	manualset3
142415	11	408884	5	NULL	NULL	0	NULL	Face-to-face interviews	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors draw on social support theory to examine supervisor support match ( support wanted and received ) , support mismatch ( support not wanted and received ) and work outcomes for abused low-wage working women , and to determine if supervisor support match and mismatch are more strongly associated with work outcomes than global supervisor support Face-to-face interviews were conducted with a community sample of abused , employed women who have experienced intimate partner violence ( IPV ) in the past year ( N = 163 ) .
	manualset3
142416	12	408884	5	NULL	NULL	0	NULL	community sample	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors draw on social support theory to examine supervisor support match ( support wanted and received ) , support mismatch ( support not wanted and received ) and work outcomes for abused low-wage working women , and to determine if supervisor support match and mismatch are more strongly associated with work outcomes than global supervisor support Face-to-face interviews were conducted with a community sample of abused , employed women who have experienced intimate partner violence ( IPV ) in the past year ( N = 163 ) .
	manualset3
142417	13	408884	5	NULL	NULL	0	NULL	abused , employed women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors draw on social support theory to examine supervisor support match ( support wanted and received ) , support mismatch ( support not wanted and received ) and work outcomes for abused low-wage working women , and to determine if supervisor support match and mismatch are more strongly associated with work outcomes than global supervisor support Face-to-face interviews were conducted with a community sample of abused , employed women who have experienced intimate partner violence ( IPV ) in the past year ( N = 163 ) .
	manualset3
142418	14	408884	5	NULL	NULL	0	NULL	intimate partner violence ( IPV )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors draw on social support theory to examine supervisor support match ( support wanted and received ) , support mismatch ( support not wanted and received ) and work outcomes for abused low-wage working women , and to determine if supervisor support match and mismatch are more strongly associated with work outcomes than global supervisor support Face-to-face interviews were conducted with a community sample of abused , employed women who have experienced intimate partner violence ( IPV ) in the past year ( N = 163 ) .
	manualset3
142419	15	408884	5	NULL	NULL	0	NULL	past year	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors draw on social support theory to examine supervisor support match ( support wanted and received ) , support mismatch ( support not wanted and received ) and work outcomes for abused low-wage working women , and to determine if supervisor support match and mismatch are more strongly associated with work outcomes than global supervisor support Face-to-face interviews were conducted with a community sample of abused , employed women who have experienced intimate partner violence ( IPV ) in the past year ( N = 163 ) .
	manualset3
142420	16	408884	5	NULL	NULL	0	NULL	N = 163	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors draw on social support theory to examine supervisor support match ( support wanted and received ) , support mismatch ( support not wanted and received ) and work outcomes for abused low-wage working women , and to determine if supervisor support match and mismatch are more strongly associated with work outcomes than global supervisor support Face-to-face interviews were conducted with a community sample of abused , employed women who have experienced intimate partner violence ( IPV ) in the past year ( N = 163 ) .
	manualset3
142421	1	408885	5	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors examined daytime napping and nighttime sleeping durations , reported in 1996-1997 by 220 , 934 US NIH-AARP Diet and Health Study participants , in relation to Parkinson disease diagnoses at 3 clinical stages : established ( cases diagnosed before 1995 , n = 267 ) , recent ( 1995-1999 , n = 396 ) , and prediagnostic ( 2000 and after , n = 770 ) .
	manualset3
142422	2	408885	5	NULL	NULL	0	NULL	daytime napping duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors examined daytime napping and nighttime sleeping durations , reported in 1996-1997 by 220 , 934 US NIH-AARP Diet and Health Study participants , in relation to Parkinson disease diagnoses at 3 clinical stages : established ( cases diagnosed before 1995 , n = 267 ) , recent ( 1995-1999 , n = 396 ) , and prediagnostic ( 2000 and after , n = 770 ) .
	manualset3
142423	3	408885	5	NULL	NULL	0	NULL	nighttime sleeping durations	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors examined daytime napping and nighttime sleeping durations , reported in 1996-1997 by 220 , 934 US NIH-AARP Diet and Health Study participants , in relation to Parkinson disease diagnoses at 3 clinical stages : established ( cases diagnosed before 1995 , n = 267 ) , recent ( 1995-1999 , n = 396 ) , and prediagnostic ( 2000 and after , n = 770 ) .
	manualset3
142424	4	408885	5	NULL	NULL	0	NULL	1996-1997	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors examined daytime napping and nighttime sleeping durations , reported in 1996-1997 by 220 , 934 US NIH-AARP Diet and Health Study participants , in relation to Parkinson disease diagnoses at 3 clinical stages : established ( cases diagnosed before 1995 , n = 267 ) , recent ( 1995-1999 , n = 396 ) , and prediagnostic ( 2000 and after , n = 770 ) .
	manualset3
142425	5	408885	5	NULL	NULL	0	NULL	220	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors examined daytime napping and nighttime sleeping durations , reported in 1996-1997 by 220 , 934 US NIH-AARP Diet and Health Study participants , in relation to Parkinson disease diagnoses at 3 clinical stages : established ( cases diagnosed before 1995 , n = 267 ) , recent ( 1995-1999 , n = 396 ) , and prediagnostic ( 2000 and after , n = 770 ) .
	manualset3
142426	6	408885	5	NULL	NULL	0	NULL	934 US NIH-AARP Diet and Health Study participants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors examined daytime napping and nighttime sleeping durations , reported in 1996-1997 by 220 , 934 US NIH-AARP Diet and Health Study participants , in relation to Parkinson disease diagnoses at 3 clinical stages : established ( cases diagnosed before 1995 , n = 267 ) , recent ( 1995-1999 , n = 396 ) , and prediagnostic ( 2000 and after , n = 770 ) .
	manualset3
142427	7	408885	5	NULL	NULL	0	NULL	Parkinson disease diagnoses	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors examined daytime napping and nighttime sleeping durations , reported in 1996-1997 by 220 , 934 US NIH-AARP Diet and Health Study participants , in relation to Parkinson disease diagnoses at 3 clinical stages : established ( cases diagnosed before 1995 , n = 267 ) , recent ( 1995-1999 , n = 396 ) , and prediagnostic ( 2000 and after , n = 770 ) .
	manualset3
142428	8	408885	5	NULL	NULL	0	NULL	3 clinical stages	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors examined daytime napping and nighttime sleeping durations , reported in 1996-1997 by 220 , 934 US NIH-AARP Diet and Health Study participants , in relation to Parkinson disease diagnoses at 3 clinical stages : established ( cases diagnosed before 1995 , n = 267 ) , recent ( 1995-1999 , n = 396 ) , and prediagnostic ( 2000 and after , n = 770 ) .
	manualset3
142429	9	408885	5	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors examined daytime napping and nighttime sleeping durations , reported in 1996-1997 by 220 , 934 US NIH-AARP Diet and Health Study participants , in relation to Parkinson disease diagnoses at 3 clinical stages : established ( cases diagnosed before 1995 , n = 267 ) , recent ( 1995-1999 , n = 396 ) , and prediagnostic ( 2000 and after , n = 770 ) .
	manualset3
142430	10	408885	5	NULL	NULL	0	NULL	1995	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors examined daytime napping and nighttime sleeping durations , reported in 1996-1997 by 220 , 934 US NIH-AARP Diet and Health Study participants , in relation to Parkinson disease diagnoses at 3 clinical stages : established ( cases diagnosed before 1995 , n = 267 ) , recent ( 1995-1999 , n = 396 ) , and prediagnostic ( 2000 and after , n = 770 ) .
	manualset3
142431	11	408885	5	NULL	NULL	0	NULL	n = 267	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors examined daytime napping and nighttime sleeping durations , reported in 1996-1997 by 220 , 934 US NIH-AARP Diet and Health Study participants , in relation to Parkinson disease diagnoses at 3 clinical stages : established ( cases diagnosed before 1995 , n = 267 ) , recent ( 1995-1999 , n = 396 ) , and prediagnostic ( 2000 and after , n = 770 ) .
	manualset3
142432	12	408885	5	NULL	NULL	0	NULL	1995-1999	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors examined daytime napping and nighttime sleeping durations , reported in 1996-1997 by 220 , 934 US NIH-AARP Diet and Health Study participants , in relation to Parkinson disease diagnoses at 3 clinical stages : established ( cases diagnosed before 1995 , n = 267 ) , recent ( 1995-1999 , n = 396 ) , and prediagnostic ( 2000 and after , n = 770 ) .
	manualset3
142433	13	408885	5	NULL	NULL	0	NULL	n = 396	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors examined daytime napping and nighttime sleeping durations , reported in 1996-1997 by 220 , 934 US NIH-AARP Diet and Health Study participants , in relation to Parkinson disease diagnoses at 3 clinical stages : established ( cases diagnosed before 1995 , n = 267 ) , recent ( 1995-1999 , n = 396 ) , and prediagnostic ( 2000 and after , n = 770 ) .
	manualset3
142434	14	408885	5	NULL	NULL	NULL	NULL	2000 and after	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The authors examined daytime napping and nighttime sleeping durations , reported in 1996-1997 by 220 , 934 US NIH-AARP Diet and Health Study participants , in relation to Parkinson disease diagnoses at 3 clinical stages : established ( cases diagnosed before 1995 , n = 267 ) , recent ( 1995-1999 , n = 396 ) , and prediagnostic ( 2000 and after , n = 770 ) .
	manualset3
142435	15	408885	5	NULL	NULL	0	NULL	n = 770	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors examined daytime napping and nighttime sleeping durations , reported in 1996-1997 by 220 , 934 US NIH-AARP Diet and Health Study participants , in relation to Parkinson disease diagnoses at 3 clinical stages : established ( cases diagnosed before 1995 , n = 267 ) , recent ( 1995-1999 , n = 396 ) , and prediagnostic ( 2000 and after , n = 770 ) .
	manualset3
142436	1	408886	5	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors have developed a Haddon matrix to identify factors that increase the risk of fatal rather than non-fatal pesticide self-poisoning in Sri Lanka .
	manualset3
142437	2	408886	5	NULL	NULL	0	NULL	Haddon matrix	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors have developed a Haddon matrix to identify factors that increase the risk of fatal rather than non-fatal pesticide self-poisoning in Sri Lanka .
	manualset3
142438	3	408886	5	NULL	NULL	0	NULL	factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors have developed a Haddon matrix to identify factors that increase the risk of fatal rather than non-fatal pesticide self-poisoning in Sri Lanka .
	manualset3
142440	5	408886	5	NULL	NULL	0	NULL	risk	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors have developed a Haddon matrix to identify factors that increase the risk of fatal rather than non-fatal pesticide self-poisoning in Sri Lanka .
	manualset3
142441	6	408886	5	NULL	NULL	0	NULL	pesticide self-poisoning 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors have developed a Haddon matrix to identify factors that increase the risk of fatal rather than non-fatal pesticide self-poisoning in Sri Lanka .
	manualset3
142442	7	408886	5	NULL	NULL	0	NULL	Sri Lanka	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors have developed a Haddon matrix to identify factors that increase the risk of fatal rather than non-fatal pesticide self-poisoning in Sri Lanka .
	manualset3
142443	1	408887	5	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors investigate the peculiar nature of the outbreak and find that they can not easily explain the apparent age and gender bias .
	manualset3
142444	2	408887	5	NULL	NULL	0	NULL	peculiar nature	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors investigate the peculiar nature of the outbreak and find that they can not easily explain the apparent age and gender bias .
	manualset3
142445	3	408887	5	NULL	NULL	0	NULL	outbreak	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors investigate the peculiar nature of the outbreak and find that they can not easily explain the apparent age and gender bias .
	manualset3
142446	4	408887	5	NULL	NULL	0	NULL	age	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors investigate the peculiar nature of the outbreak and find that they can not easily explain the apparent age and gender bias .
	manualset3
142447	5	408887	5	NULL	NULL	0	NULL	gender bias	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors investigate the peculiar nature of the outbreak and find that they can not easily explain the apparent age and gender bias .
	manualset3
142448	1	408888	5	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors investigated three types of implants : 1 .
	manualset3
142449	2	408888	5	NULL	NULL	0	NULL	three types	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors investigated three types of implants : 1 .
	manualset3
142450	3	408888	5	NULL	NULL	0	NULL	implants	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors investigated three types of implants : 1 .
	manualset3
142451	1	408889	5	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors investigated in 25 patients with luxations of the patella if an increased incidence of defective torsions of the leg skeleton could be demonstrated .
	manualset3
142452	2	408889	5	NULL	NULL	0	NULL	25 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors investigated in 25 patients with luxations of the patella if an increased incidence of defective torsions of the leg skeleton could be demonstrated .
	manualset3
142453	3	408889	5	NULL	NULL	NULL	NULL	luxations 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The authors investigated in 25 patients with luxations of the patella if an increased incidence of defective torsions of the leg skeleton could be demonstrated .
	manualset3
142454	4	408889	5	NULL	NULL	0	NULL	patella 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors investigated in 25 patients with luxations of the patella if an increased incidence of defective torsions of the leg skeleton could be demonstrated .
	manualset3
142455	5	408889	5	NULL	NULL	0	NULL	increased incidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors investigated in 25 patients with luxations of the patella if an increased incidence of defective torsions of the leg skeleton could be demonstrated .
	manualset3
142456	6	408889	5	NULL	NULL	0	NULL	defective torsions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors investigated in 25 patients with luxations of the patella if an increased incidence of defective torsions of the leg skeleton could be demonstrated .
	manualset3
142457	7	408889	5	NULL	NULL	0	NULL	leg skeleton	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors investigated in 25 patients with luxations of the patella if an increased incidence of defective torsions of the leg skeleton could be demonstrated .
	manualset3
142458	1	408890	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors of this study present a literature review and report a case of nasal histoplasmosis in a patient with AIDS .
	manualset3
142459	2	408890	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors of this study present a literature review and report a case of nasal histoplasmosis in a patient with AIDS .
	manualset3
142460	3	408890	5	NULL	NULL	0	NULL	literature review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors of this study present a literature review and report a case of nasal histoplasmosis in a patient with AIDS .
	manualset3
142461	4	408890	5	NULL	NULL	0	NULL	case 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors of this study present a literature review and report a case of nasal histoplasmosis in a patient with AIDS .
	manualset3
142462	5	408890	5	NULL	NULL	0	NULL	nasal histoplasmosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors of this study present a literature review and report a case of nasal histoplasmosis in a patient with AIDS .
	manualset3
142463	6	408890	5	NULL	NULL	0	NULL	patient 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors of this study present a literature review and report a case of nasal histoplasmosis in a patient with AIDS .
	manualset3
142464	7	408890	5	NULL	NULL	0	NULL	AIDS 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors of this study present a literature review and report a case of nasal histoplasmosis in a patient with AIDS .
	manualset3
142465	1	408891	5	NULL	NULL	0	NULL	second mouse model ( Fxr1 + neo )	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A second mouse model ( Fxr1 + neo ) , which expresses strongly reduced levels of Fxr1p relative to WT littermates , does not display the neonatal lethal phenotype seen in the Fxr1 KOs but does display a strongly reduced limb musculature and has a reduced life span of approximately 18 weeks .
	manualset3
142466	2	408891	5	NULL	NULL	0	NULL	levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A second mouse model ( Fxr1 + neo ) , which expresses strongly reduced levels of Fxr1p relative to WT littermates , does not display the neonatal lethal phenotype seen in the Fxr1 KOs but does display a strongly reduced limb musculature and has a reduced life span of approximately 18 weeks .
	manualset3
142467	3	408891	5	NULL	NULL	0	NULL	Fxr1p 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A second mouse model ( Fxr1 + neo ) , which expresses strongly reduced levels of Fxr1p relative to WT littermates , does not display the neonatal lethal phenotype seen in the Fxr1 KOs but does display a strongly reduced limb musculature and has a reduced life span of approximately 18 weeks .
	manualset3
142468	4	408891	5	NULL	NULL	0	NULL	WT littermates 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A second mouse model ( Fxr1 + neo ) , which expresses strongly reduced levels of Fxr1p relative to WT littermates , does not display the neonatal lethal phenotype seen in the Fxr1 KOs but does display a strongly reduced limb musculature and has a reduced life span of approximately 18 weeks .
	manualset3
142469	5	408891	5	NULL	NULL	0	NULL	neonatal lethal phenotype	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A second mouse model ( Fxr1 + neo ) , which expresses strongly reduced levels of Fxr1p relative to WT littermates , does not display the neonatal lethal phenotype seen in the Fxr1 KOs but does display a strongly reduced limb musculature and has a reduced life span of approximately 18 weeks .
	manualset3
142470	6	408891	5	NULL	NULL	0	NULL	Fxr1 KOs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A second mouse model ( Fxr1 + neo ) , which expresses strongly reduced levels of Fxr1p relative to WT littermates , does not display the neonatal lethal phenotype seen in the Fxr1 KOs but does display a strongly reduced limb musculature and has a reduced life span of approximately 18 weeks .
	manualset3
142471	7	408891	5	NULL	NULL	0	NULL	limb musculature	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A second mouse model ( Fxr1 + neo ) , which expresses strongly reduced levels of Fxr1p relative to WT littermates , does not display the neonatal lethal phenotype seen in the Fxr1 KOs but does display a strongly reduced limb musculature and has a reduced life span of approximately 18 weeks .
	manualset3
142472	8	408891	5	NULL	NULL	0	NULL	reduced life span	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A second mouse model ( Fxr1 + neo ) , which expresses strongly reduced levels of Fxr1p relative to WT littermates , does not display the neonatal lethal phenotype seen in the Fxr1 KOs but does display a strongly reduced limb musculature and has a reduced life span of approximately 18 weeks .
	manualset3
142473	9	408891	5	NULL	NULL	0	NULL	18 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A second mouse model ( Fxr1 + neo ) , which expresses strongly reduced levels of Fxr1p relative to WT littermates , does not display the neonatal lethal phenotype seen in the Fxr1 KOs but does display a strongly reduced limb musculature and has a reduced life span of approximately 18 weeks .
	manualset3
142474	1	408892	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors present the case of a 2 years old girl , first diagnosed with enterocolitis , but her clinical evolution revealed a complex situation : both celiac disease and secondary lactose intolerance .
	manualset3
142475	2	408892	5	NULL	NULL	0	NULL	case 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors present the case of a 2 years old girl , first diagnosed with enterocolitis , but her clinical evolution revealed a complex situation : both celiac disease and secondary lactose intolerance .
	manualset3
142476	3	408892	5	NULL	NULL	0	NULL	2 years old girl 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors present the case of a 2 years old girl , first diagnosed with enterocolitis , but her clinical evolution revealed a complex situation : both celiac disease and secondary lactose intolerance .
	manualset3
142477	4	408892	5	NULL	NULL	0	NULL	enterocolitis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors present the case of a 2 years old girl , first diagnosed with enterocolitis , but her clinical evolution revealed a complex situation : both celiac disease and secondary lactose intolerance .
	manualset3
142478	5	408892	5	NULL	NULL	0	NULL	clinical evolution	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors present the case of a 2 years old girl , first diagnosed with enterocolitis , but her clinical evolution revealed a complex situation : both celiac disease and secondary lactose intolerance .
	manualset3
142479	6	408892	5	NULL	NULL	0	NULL	complex situation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors present the case of a 2 years old girl , first diagnosed with enterocolitis , but her clinical evolution revealed a complex situation : both celiac disease and secondary lactose intolerance .
	manualset3
142480	7	408892	5	NULL	NULL	0	NULL	celiac disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors present the case of a 2 years old girl , first diagnosed with enterocolitis , but her clinical evolution revealed a complex situation : both celiac disease and secondary lactose intolerance .
	manualset3
142481	8	408892	5	NULL	NULL	0	NULL	secondary lactose intolerance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors present the case of a 2 years old girl , first diagnosed with enterocolitis , but her clinical evolution revealed a complex situation : both celiac disease and secondary lactose intolerance .
	manualset3
142482	1	408893	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors present their procedure of hepaticojejunal anastomosis without suture , which is adequate for the treatment of benign or even malignant stenosis of the CBD .
	manualset3
142483	2	408893	5	NULL	NULL	0	NULL	procedure of hepaticojejunal anastomosis without suture	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors present their procedure of hepaticojejunal anastomosis without suture , which is adequate for the treatment of benign or even malignant stenosis of the CBD .
	manualset3
142484	3	408893	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors present their procedure of hepaticojejunal anastomosis without suture , which is adequate for the treatment of benign or even malignant stenosis of the CBD .
	manualset3
142485	4	408893	5	NULL	NULL	0	NULL	benign or even malignant stenosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors present their procedure of hepaticojejunal anastomosis without suture , which is adequate for the treatment of benign or even malignant stenosis of the CBD .
	manualset3
142486	5	408893	5	NULL	NULL	0	NULL	CBD 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors present their procedure of hepaticojejunal anastomosis without suture , which is adequate for the treatment of benign or even malignant stenosis of the CBD .
	manualset3
142487	1	408894	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors propose that 1 month after a 1-hour exposure to chrysotile asbestos , fiber-induced membrane injury in cells of the lung interstitium leads to formation of microcalcifications .
	manualset3
142488	2	408894	5	NULL	NULL	0	NULL	1 month 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors propose that 1 month after a 1-hour exposure to chrysotile asbestos , fiber-induced membrane injury in cells of the lung interstitium leads to formation of microcalcifications .
	manualset3
142489	3	408894	5	NULL	NULL	0	NULL	1-hour exposure 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors propose that 1 month after a 1-hour exposure to chrysotile asbestos , fiber-induced membrane injury in cells of the lung interstitium leads to formation of microcalcifications .
	manualset3
142490	4	408894	5	NULL	NULL	0	NULL	chrysotile asbestos	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors propose that 1 month after a 1-hour exposure to chrysotile asbestos , fiber-induced membrane injury in cells of the lung interstitium leads to formation of microcalcifications .
	manualset3
142491	5	408894	5	NULL	NULL	0	NULL	fiber-induced membrane injury 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors propose that 1 month after a 1-hour exposure to chrysotile asbestos , fiber-induced membrane injury in cells of the lung interstitium leads to formation of microcalcifications .
	manualset3
142492	6	408894	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors propose that 1 month after a 1-hour exposure to chrysotile asbestos , fiber-induced membrane injury in cells of the lung interstitium leads to formation of microcalcifications .
	manualset3
142493	7	408894	5	NULL	NULL	0	NULL	lung interstitium	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors propose that 1 month after a 1-hour exposure to chrysotile asbestos , fiber-induced membrane injury in cells of the lung interstitium leads to formation of microcalcifications .
	manualset3
142494	8	408894	5	NULL	NULL	0	NULL	formation of microcalcifications	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors propose that 1 month after a 1-hour exposure to chrysotile asbestos , fiber-induced membrane injury in cells of the lung interstitium leads to formation of microcalcifications .
	manualset3
142495	1	408895	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors provide a detailed review of the extant gene-environment interaction ( GxE ) research in the etiology of posttraumatic stress disorder ( PTSD ) .
	manualset3
142496	2	408895	5	NULL	NULL	0	NULL	detailed review 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors provide a detailed review of the extant gene-environment interaction ( GxE ) research in the etiology of posttraumatic stress disorder ( PTSD ) .
	manualset3
142497	3	408895	5	NULL	NULL	0	NULL	extant gene-environment interaction ( GxE ) research 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors provide a detailed review of the extant gene-environment interaction ( GxE ) research in the etiology of posttraumatic stress disorder ( PTSD ) .
	manualset3
142498	4	408895	5	NULL	NULL	0	NULL	etiology 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors provide a detailed review of the extant gene-environment interaction ( GxE ) research in the etiology of posttraumatic stress disorder ( PTSD ) .
	manualset3
142499	5	408895	5	NULL	NULL	0	NULL	posttraumatic stress disorder ( PTSD ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors provide a detailed review of the extant gene-environment interaction ( GxE ) research in the etiology of posttraumatic stress disorder ( PTSD ) .
	manualset3
142500	1	408896	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors report an intrinsic brainstem lesion that was diagnosed initially as a pontine cavernoma , which finally proved to be a choroid plexus papilloma .
	manualset3
142501	2	408896	5	NULL	NULL	0	NULL	intrinsic brainstem lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors report an intrinsic brainstem lesion that was diagnosed initially as a pontine cavernoma , which finally proved to be a choroid plexus papilloma .
	manualset3
142502	3	408896	5	NULL	NULL	0	NULL	pontine cavernoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors report an intrinsic brainstem lesion that was diagnosed initially as a pontine cavernoma , which finally proved to be a choroid plexus papilloma .
	manualset3
142503	4	408896	5	NULL	NULL	0	NULL	choroid plexus papilloma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors report an intrinsic brainstem lesion that was diagnosed initially as a pontine cavernoma , which finally proved to be a choroid plexus papilloma .
	manualset3
142504	1	408897	5	NULL	NULL	NULL	NULL	authors	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The authors report on studies of the hemolytic effects of diaphenylsulfone ( DDS ) administered orally , in doses ranging from 25 mg to 300 mg daily for 21 days , to normal healthy men and to healthy Negro men with deficiency of glucose-6-phosphate dehydrogenase ( G-6-PD ) .
	manualset3
142505	2	408897	5	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors report on studies of the hemolytic effects of diaphenylsulfone ( DDS ) administered orally , in doses ranging from 25 mg to 300 mg daily for 21 days , to normal healthy men and to healthy Negro men with deficiency of glucose-6-phosphate dehydrogenase ( G-6-PD ) .
	manualset3
142506	3	408897	5	NULL	NULL	0	NULL	hemolytic effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors report on studies of the hemolytic effects of diaphenylsulfone ( DDS ) administered orally , in doses ranging from 25 mg to 300 mg daily for 21 days , to normal healthy men and to healthy Negro men with deficiency of glucose-6-phosphate dehydrogenase ( G-6-PD ) .
	manualset3
142507	4	408897	5	NULL	NULL	0	NULL	diaphenylsulfone ( DDS ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors report on studies of the hemolytic effects of diaphenylsulfone ( DDS ) administered orally , in doses ranging from 25 mg to 300 mg daily for 21 days , to normal healthy men and to healthy Negro men with deficiency of glucose-6-phosphate dehydrogenase ( G-6-PD ) .
	manualset3
142508	5	408897	5	NULL	NULL	0	NULL	doses 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors report on studies of the hemolytic effects of diaphenylsulfone ( DDS ) administered orally , in doses ranging from 25 mg to 300 mg daily for 21 days , to normal healthy men and to healthy Negro men with deficiency of glucose-6-phosphate dehydrogenase ( G-6-PD ) .
	manualset3
142509	6	408897	5	NULL	NULL	0	NULL	25 mg to 300 mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors report on studies of the hemolytic effects of diaphenylsulfone ( DDS ) administered orally , in doses ranging from 25 mg to 300 mg daily for 21 days , to normal healthy men and to healthy Negro men with deficiency of glucose-6-phosphate dehydrogenase ( G-6-PD ) .
	manualset3
142510	7	408897	5	NULL	NULL	0	NULL	21 days 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors report on studies of the hemolytic effects of diaphenylsulfone ( DDS ) administered orally , in doses ranging from 25 mg to 300 mg daily for 21 days , to normal healthy men and to healthy Negro men with deficiency of glucose-6-phosphate dehydrogenase ( G-6-PD ) .
	manualset3
142511	8	408897	5	NULL	NULL	0	NULL	normal healthy men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors report on studies of the hemolytic effects of diaphenylsulfone ( DDS ) administered orally , in doses ranging from 25 mg to 300 mg daily for 21 days , to normal healthy men and to healthy Negro men with deficiency of glucose-6-phosphate dehydrogenase ( G-6-PD ) .
	manualset3
142512	9	408897	5	NULL	NULL	0	NULL	healthy Negro men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors report on studies of the hemolytic effects of diaphenylsulfone ( DDS ) administered orally , in doses ranging from 25 mg to 300 mg daily for 21 days , to normal healthy men and to healthy Negro men with deficiency of glucose-6-phosphate dehydrogenase ( G-6-PD ) .
	manualset3
142513	10	408897	5	NULL	NULL	0	NULL	deficiency 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors report on studies of the hemolytic effects of diaphenylsulfone ( DDS ) administered orally , in doses ranging from 25 mg to 300 mg daily for 21 days , to normal healthy men and to healthy Negro men with deficiency of glucose-6-phosphate dehydrogenase ( G-6-PD ) .
	manualset3
142514	11	408897	5	NULL	NULL	0	NULL	glucose-6-phosphate dehydrogenase ( G-6-PD )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors report on studies of the hemolytic effects of diaphenylsulfone ( DDS ) administered orally , in doses ranging from 25 mg to 300 mg daily for 21 days , to normal healthy men and to healthy Negro men with deficiency of glucose-6-phosphate dehydrogenase ( G-6-PD ) .
	manualset3
142515	1	408898	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors report the case of a 27-year-old woman with gamma probe-guided resection of a recurrent regional lymph node metastasis in papillary thyroid cancer .
	manualset3
142516	2	408898	5	NULL	NULL	0	NULL	case 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors report the case of a 27-year-old woman with gamma probe-guided resection of a recurrent regional lymph node metastasis in papillary thyroid cancer .
	manualset3
142517	3	408898	5	NULL	NULL	0	NULL	27-year-old woman	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors report the case of a 27-year-old woman with gamma probe-guided resection of a recurrent regional lymph node metastasis in papillary thyroid cancer .
	manualset3
142518	4	408898	5	NULL	NULL	0	NULL	gamma probe-guided resection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors report the case of a 27-year-old woman with gamma probe-guided resection of a recurrent regional lymph node metastasis in papillary thyroid cancer .
	manualset3
142519	5	408898	5	NULL	NULL	0	NULL	recurrent regional lymph node metastasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors report the case of a 27-year-old woman with gamma probe-guided resection of a recurrent regional lymph node metastasis in papillary thyroid cancer .
	manualset3
142520	6	408898	5	NULL	NULL	0	NULL	papillary thyroid cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors report the case of a 27-year-old woman with gamma probe-guided resection of a recurrent regional lymph node metastasis in papillary thyroid cancer .
	manualset3
142521	1	408899	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors report the first case of prosthetic valve endocarditis caused by Gemella sanguinis .
	manualset3
142522	2	408899	5	NULL	NULL	0	NULL	first case	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors report the first case of prosthetic valve endocarditis caused by Gemella sanguinis .
	manualset3
142523	3	408899	5	NULL	NULL	0	NULL	prosthetic valve endocarditis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors report the first case of prosthetic valve endocarditis caused by Gemella sanguinis .
	manualset3
142524	4	408899	5	NULL	NULL	0	NULL	Gemella sanguinis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors report the first case of prosthetic valve endocarditis caused by Gemella sanguinis .
	manualset3
142525	1	408900	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors reviewed cohort and case-control studies that reported on the association between abnormal hip morphology and hip OA .
	manualset3
142526	2	408900	5	NULL	NULL	0	NULL	cohort studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors reviewed cohort and case-control studies that reported on the association between abnormal hip morphology and hip OA .
	manualset3
142527	3	408900	5	NULL	NULL	0	NULL	case-control studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors reviewed cohort and case-control studies that reported on the association between abnormal hip morphology and hip OA .
	manualset3
142528	4	408900	5	NULL	NULL	0	NULL	association 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors reviewed cohort and case-control studies that reported on the association between abnormal hip morphology and hip OA .
	manualset3
142529	5	408900	5	NULL	NULL	0	NULL	abnormal hip morphology 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors reviewed cohort and case-control studies that reported on the association between abnormal hip morphology and hip OA .
	manualset3
142530	6	408900	5	NULL	NULL	0	NULL	hip OA	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors reviewed cohort and case-control studies that reported on the association between abnormal hip morphology and hip OA .
	manualset3
142531	1	408901	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors reviewed the literature regarding chemotherapeutic agents given during the first trimester of pregnancy .
	manualset3
142532	2	408901	5	NULL	NULL	0	NULL	literature 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors reviewed the literature regarding chemotherapeutic agents given during the first trimester of pregnancy .
	manualset3
142533	3	408901	5	NULL	NULL	0	NULL	chemotherapeutic agents	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors reviewed the literature regarding chemotherapeutic agents given during the first trimester of pregnancy .
	manualset3
142534	4	408901	5	NULL	NULL	0	NULL	first trimester of pregnancy	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors reviewed the literature regarding chemotherapeutic agents given during the first trimester of pregnancy .
	manualset3
142535	1	408902	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors routinely implement prophylactic antibiotic coverage with doxycycline 100 mg every 12 hours for vibrio in patients with wounds exposed to or acquired in saltwater .
	manualset3
142536	2	408902	5	NULL	NULL	0	NULL	prophylactic antibiotic coverage 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors routinely implement prophylactic antibiotic coverage with doxycycline 100 mg every 12 hours for vibrio in patients with wounds exposed to or acquired in saltwater .
	manualset3
142537	3	408902	5	NULL	NULL	0	NULL	doxycycline	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors routinely implement prophylactic antibiotic coverage with doxycycline 100 mg every 12 hours for vibrio in patients with wounds exposed to or acquired in saltwater .
	manualset3
142538	4	408902	5	NULL	NULL	0	NULL	100 mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors routinely implement prophylactic antibiotic coverage with doxycycline 100 mg every 12 hours for vibrio in patients with wounds exposed to or acquired in saltwater .
	manualset3
142539	5	408902	5	NULL	NULL	0	NULL	 12 hours 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors routinely implement prophylactic antibiotic coverage with doxycycline 100 mg every 12 hours for vibrio in patients with wounds exposed to or acquired in saltwater .
	manualset3
142540	6	408902	5	NULL	NULL	0	NULL	vibrio 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors routinely implement prophylactic antibiotic coverage with doxycycline 100 mg every 12 hours for vibrio in patients with wounds exposed to or acquired in saltwater .
	manualset3
142541	7	408902	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors routinely implement prophylactic antibiotic coverage with doxycycline 100 mg every 12 hours for vibrio in patients with wounds exposed to or acquired in saltwater .
	manualset3
142542	8	408902	5	NULL	NULL	0	NULL	wounds 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors routinely implement prophylactic antibiotic coverage with doxycycline 100 mg every 12 hours for vibrio in patients with wounds exposed to or acquired in saltwater .
	manualset3
142543	9	408902	5	NULL	NULL	0	NULL	saltwater 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors routinely implement prophylactic antibiotic coverage with doxycycline 100 mg every 12 hours for vibrio in patients with wounds exposed to or acquired in saltwater .
	manualset3
142544	1	408903	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors sought to compare the antiemetic and sedative postanesthetic effects of droperidol versus lidocaine given intravenously .
	manualset3
142545	2	408903	5	NULL	NULL	0	NULL	antiemetic effect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors sought to compare the antiemetic and sedative postanesthetic effects of droperidol versus lidocaine given intravenously .
	manualset3
142546	3	408903	5	NULL	NULL	0	NULL	sedative postanesthetic effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors sought to compare the antiemetic and sedative postanesthetic effects of droperidol versus lidocaine given intravenously .
	manualset3
142547	4	408903	5	NULL	NULL	0	NULL	droperidol 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors sought to compare the antiemetic and sedative postanesthetic effects of droperidol versus lidocaine given intravenously .
	manualset3
142548	5	408903	5	NULL	NULL	0	NULL	lidocaine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors sought to compare the antiemetic and sedative postanesthetic effects of droperidol versus lidocaine given intravenously .
	manualset3
142549	1	408904	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors suggest actions for nurse administrators and researchers who must address frequent queries as to the adequacy of nursing staffing .
	manualset3
142550	2	408904	5	NULL	NULL	0	NULL	actions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors suggest actions for nurse administrators and researchers who must address frequent queries as to the adequacy of nursing staffing .
	manualset3
142551	3	408904	5	NULL	NULL	0	NULL	nurse administrators	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors suggest actions for nurse administrators and researchers who must address frequent queries as to the adequacy of nursing staffing .
	manualset3
142552	4	408904	5	NULL	NULL	0	NULL	researchers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors suggest actions for nurse administrators and researchers who must address frequent queries as to the adequacy of nursing staffing .
	manualset3
142553	5	408904	5	NULL	NULL	0	NULL	queries 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors suggest actions for nurse administrators and researchers who must address frequent queries as to the adequacy of nursing staffing .
	manualset3
142554	6	408904	5	NULL	NULL	0	NULL	adequacy 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors suggest actions for nurse administrators and researchers who must address frequent queries as to the adequacy of nursing staffing .
	manualset3
147966	7	408904	5	NULL	NULL	0	NULL	nursing staffing	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors suggest actions for nurse administrators and researchers who must address frequent queries as to the adequacy of nursing staffing .
	manualset3
142555	1	408905	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors suggest that clonazepam is a safe and effective medication in the treatment of social phobia .
	manualset3
142556	2	408905	5	NULL	NULL	0	NULL	clonazepam 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors suggest that clonazepam is a safe and effective medication in the treatment of social phobia .
	manualset3
142557	3	408905	5	NULL	NULL	0	NULL	medication 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors suggest that clonazepam is a safe and effective medication in the treatment of social phobia .
	manualset3
142558	4	408905	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors suggest that clonazepam is a safe and effective medication in the treatment of social phobia .
	manualset3
142559	5	408905	5	NULL	NULL	0	NULL	social phobia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors suggest that clonazepam is a safe and effective medication in the treatment of social phobia .
	manualset3
142560	1	408906	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors suggest that in HIV-positive patients who present with spinal lesions , KS should be included in the differential diagnosis .
	manualset3
142561	2	408906	5	NULL	NULL	0	NULL	HIV-positive patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors suggest that in HIV-positive patients who present with spinal lesions , KS should be included in the differential diagnosis .
	manualset3
142562	3	408906	5	NULL	NULL	0	NULL	spinal lesions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors suggest that in HIV-positive patients who present with spinal lesions , KS should be included in the differential diagnosis .
	manualset3
142563	4	408906	5	NULL	NULL	0	NULL	KS 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors suggest that in HIV-positive patients who present with spinal lesions , KS should be included in the differential diagnosis .
	manualset3
142564	5	408906	5	NULL	NULL	0	NULL	differential diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors suggest that in HIV-positive patients who present with spinal lesions , KS should be included in the differential diagnosis .
	manualset3
142565	1	408907	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors summarize results of multiyear investigations at the Institute of Biomedical Problems of induced motion sickness and development of prophylactic medicaments representing various classes of biologically active substances ( choline blocking agents , sympathomimetics , antihistamines etc. ) prescribed singularly or in an combination based on the knowledge of MS-provoking inter-receptor interactions and therapeutic effects of drugs .
	manualset3
142566	2	408907	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors summarize results of multiyear investigations at the Institute of Biomedical Problems of induced motion sickness and development of prophylactic medicaments representing various classes of biologically active substances ( choline blocking agents , sympathomimetics , antihistamines etc. ) prescribed singularly or in an combination based on the knowledge of MS-provoking inter-receptor interactions and therapeutic effects of drugs .
	manualset3
142568	3	408907	5	NULL	NULL	0	NULL	multiyear investigations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors summarize results of multiyear investigations at the Institute of Biomedical Problems of induced motion sickness and development of prophylactic medicaments representing various classes of biologically active substances ( choline blocking agents , sympathomimetics , antihistamines etc. ) prescribed singularly or in an combination based on the knowledge of MS-provoking inter-receptor interactions and therapeutic effects of drugs .
	manualset3
142569	4	408907	5	NULL	NULL	0	NULL	Institute of Biomedical Problems	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors summarize results of multiyear investigations at the Institute of Biomedical Problems of induced motion sickness and development of prophylactic medicaments representing various classes of biologically active substances ( choline blocking agents , sympathomimetics , antihistamines etc. ) prescribed singularly or in an combination based on the knowledge of MS-provoking inter-receptor interactions and therapeutic effects of drugs .
	manualset3
142570	5	408907	5	NULL	NULL	0	NULL	induced motion sickness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors summarize results of multiyear investigations at the Institute of Biomedical Problems of induced motion sickness and development of prophylactic medicaments representing various classes of biologically active substances ( choline blocking agents , sympathomimetics , antihistamines etc. ) prescribed singularly or in an combination based on the knowledge of MS-provoking inter-receptor interactions and therapeutic effects of drugs .
	manualset3
142571	6	408907	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors summarize results of multiyear investigations at the Institute of Biomedical Problems of induced motion sickness and development of prophylactic medicaments representing various classes of biologically active substances ( choline blocking agents , sympathomimetics , antihistamines etc. ) prescribed singularly or in an combination based on the knowledge of MS-provoking inter-receptor interactions and therapeutic effects of drugs .
	manualset3
142572	7	408907	5	NULL	NULL	0	NULL	biologically active substances	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors summarize results of multiyear investigations at the Institute of Biomedical Problems of induced motion sickness and development of prophylactic medicaments representing various classes of biologically active substances ( choline blocking agents , sympathomimetics , antihistamines etc. ) prescribed singularly or in an combination based on the knowledge of MS-provoking inter-receptor interactions and therapeutic effects of drugs .
	manualset3
142573	8	408907	5	NULL	NULL	0	NULL	choline blocking agents	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors summarize results of multiyear investigations at the Institute of Biomedical Problems of induced motion sickness and development of prophylactic medicaments representing various classes of biologically active substances ( choline blocking agents , sympathomimetics , antihistamines etc. ) prescribed singularly or in an combination based on the knowledge of MS-provoking inter-receptor interactions and therapeutic effects of drugs .
	manualset3
142574	9	408907	5	NULL	NULL	0	NULL	sympathomimetics 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors summarize results of multiyear investigations at the Institute of Biomedical Problems of induced motion sickness and development of prophylactic medicaments representing various classes of biologically active substances ( choline blocking agents , sympathomimetics , antihistamines etc. ) prescribed singularly or in an combination based on the knowledge of MS-provoking inter-receptor interactions and therapeutic effects of drugs .
	manualset3
142575	10	408907	5	NULL	NULL	0	NULL	antihistamines 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors summarize results of multiyear investigations at the Institute of Biomedical Problems of induced motion sickness and development of prophylactic medicaments representing various classes of biologically active substances ( choline blocking agents , sympathomimetics , antihistamines etc. ) prescribed singularly or in an combination based on the knowledge of MS-provoking inter-receptor interactions and therapeutic effects of drugs .
	manualset3
142576	11	408907	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors summarize results of multiyear investigations at the Institute of Biomedical Problems of induced motion sickness and development of prophylactic medicaments representing various classes of biologically active substances ( choline blocking agents , sympathomimetics , antihistamines etc. ) prescribed singularly or in an combination based on the knowledge of MS-provoking inter-receptor interactions and therapeutic effects of drugs .
	manualset3
142577	12	408907	5	NULL	NULL	0	NULL	knowledge 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors summarize results of multiyear investigations at the Institute of Biomedical Problems of induced motion sickness and development of prophylactic medicaments representing various classes of biologically active substances ( choline blocking agents , sympathomimetics , antihistamines etc. ) prescribed singularly or in an combination based on the knowledge of MS-provoking inter-receptor interactions and therapeutic effects of drugs .
	manualset3
142578	13	408907	5	NULL	NULL	0	NULL	 MS-provoking inter-receptor interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors summarize results of multiyear investigations at the Institute of Biomedical Problems of induced motion sickness and development of prophylactic medicaments representing various classes of biologically active substances ( choline blocking agents , sympathomimetics , antihistamines etc. ) prescribed singularly or in an combination based on the knowledge of MS-provoking inter-receptor interactions and therapeutic effects of drugs .
	manualset3
142579	14	408907	5	NULL	NULL	0	NULL	therapeutic effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors summarize results of multiyear investigations at the Institute of Biomedical Problems of induced motion sickness and development of prophylactic medicaments representing various classes of biologically active substances ( choline blocking agents , sympathomimetics , antihistamines etc. ) prescribed singularly or in an combination based on the knowledge of MS-provoking inter-receptor interactions and therapeutic effects of drugs .
	manualset3
142580	15	408907	5	NULL	NULL	0	NULL	drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors summarize results of multiyear investigations at the Institute of Biomedical Problems of induced motion sickness and development of prophylactic medicaments representing various classes of biologically active substances ( choline blocking agents , sympathomimetics , antihistamines etc. ) prescribed singularly or in an combination based on the knowledge of MS-provoking inter-receptor interactions and therapeutic effects of drugs .
	manualset3
142581	1	408908	5	NULL	NULL	0	NULL	secondary purpose 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A secondary purpose was to establish the contributions of pre-competition affects to post-competition performance appraisals , independent of pre-competition performance expectations .
	manualset3
142582	2	408908	5	NULL	NULL	0	NULL	contributions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A secondary purpose was to establish the contributions of pre-competition affects to post-competition performance appraisals , independent of pre-competition performance expectations .
	manualset3
142583	3	408908	5	NULL	NULL	0	NULL	pre-competition affects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A secondary purpose was to establish the contributions of pre-competition affects to post-competition performance appraisals , independent of pre-competition performance expectations .
	manualset3
142584	4	408908	5	NULL	NULL	0	NULL	post-competition performance appraisals	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A secondary purpose was to establish the contributions of pre-competition affects to post-competition performance appraisals , independent of pre-competition performance expectations .
	manualset3
142585	5	408908	5	NULL	NULL	0	NULL	pre-competition performance expectations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A secondary purpose was to establish the contributions of pre-competition affects to post-competition performance appraisals , independent of pre-competition performance expectations .
	manualset3
142586	1	408909	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors tested key hypotheses in the literature pertaining to chronic grief and resilience by identifying the preloss predictors of each pattern .
	manualset3
142587	2	408909	5	NULL	NULL	0	NULL	tested key hypotheses	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors tested key hypotheses in the literature pertaining to chronic grief and resilience by identifying the preloss predictors of each pattern .
	manualset3
142588	3	408909	5	NULL	NULL	0	NULL	literature 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors tested key hypotheses in the literature pertaining to chronic grief and resilience by identifying the preloss predictors of each pattern .
	manualset3
142589	4	408909	5	NULL	NULL	0	NULL	chronic grief 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors tested key hypotheses in the literature pertaining to chronic grief and resilience by identifying the preloss predictors of each pattern .
	manualset3
142590	5	408909	5	NULL	NULL	0	NULL	resilience 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors tested key hypotheses in the literature pertaining to chronic grief and resilience by identifying the preloss predictors of each pattern .
	manualset3
142591	6	408909	5	NULL	NULL	0	NULL	preloss predictors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors tested key hypotheses in the literature pertaining to chronic grief and resilience by identifying the preloss predictors of each pattern .
	manualset3
142592	7	408909	5	NULL	NULL	0	NULL	pattern 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors tested key hypotheses in the literature pertaining to chronic grief and resilience by identifying the preloss predictors of each pattern .
	manualset3
142593	1	408910	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors used the Turkish form of K. Bartholomew and L. M. Horowitz 's ( 1991 ) Relationship Questionnaire ( RQ ) to measure participants ' general and specific attachment orientations .
	manualset3
142594	2	408910	5	NULL	NULL	0	NULL	Turkish form	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors used the Turkish form of K. Bartholomew and L. M. Horowitz 's ( 1991 ) Relationship Questionnaire ( RQ ) to measure participants ' general and specific attachment orientations .
	manualset3
142595	3	408910	5	NULL	NULL	0	NULL	K. Bartholomew and L. M. Horowitz 's ( 1991 ) Relationship Questionnaire ( RQ ) 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors used the Turkish form of K. Bartholomew and L. M. Horowitz 's ( 1991 ) Relationship Questionnaire ( RQ ) to measure participants ' general and specific attachment orientations .
	manualset3
142596	4	408910	5	NULL	NULL	0	NULL	general orientations 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors used the Turkish form of K. Bartholomew and L. M. Horowitz 's ( 1991 ) Relationship Questionnaire ( RQ ) to measure participants ' general and specific attachment orientations .
	manualset3
142597	5	408910	5	NULL	NULL	0	NULL	specific attachment orientations 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors used the Turkish form of K. Bartholomew and L. M. Horowitz 's ( 1991 ) Relationship Questionnaire ( RQ ) to measure participants ' general and specific attachment orientations .
	manualset3
142598	1	408911	5	NULL	NULL	0	NULL	autoimmune component	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The autoimmune component of psoriasis is substantiated by multiple findings , including the isolation of activated T cells within the lesions .
	manualset3
142599	2	408911	5	NULL	NULL	0	NULL	psoriasis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The autoimmune component of psoriasis is substantiated by multiple findings , including the isolation of activated T cells within the lesions .
	manualset3
142600	3	408911	5	NULL	NULL	0	NULL	multiple findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The autoimmune component of psoriasis is substantiated by multiple findings , including the isolation of activated T cells within the lesions .
	manualset3
142601	4	408911	5	NULL	NULL	0	NULL	isolation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The autoimmune component of psoriasis is substantiated by multiple findings , including the isolation of activated T cells within the lesions .
	manualset3
142602	5	408911	5	NULL	NULL	0	NULL	activated T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The autoimmune component of psoriasis is substantiated by multiple findings , including the isolation of activated T cells within the lesions .
	manualset3
142603	6	408911	5	NULL	NULL	0	NULL	lesions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The autoimmune component of psoriasis is substantiated by multiple findings , including the isolation of activated T cells within the lesions .
	manualset3
142604	1	408912	5	NULL	NULL	0	NULL	automated full time data collection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The automated full time data collection of several different running parameters makes it also a suitable test for efficient in vivo screening of potential therapeutic compounds in this model for PD .
	manualset3
142605	2	408912	5	NULL	NULL	0	NULL	running parameters	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The automated full time data collection of several different running parameters makes it also a suitable test for efficient in vivo screening of potential therapeutic compounds in this model for PD .
	manualset3
142606	3	408912	5	NULL	NULL	NULL	NULL	suitable test	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The automated full time data collection of several different running parameters makes it also a suitable test for efficient in vivo screening of potential therapeutic compounds in this model for PD .
	manualset3
142607	4	408912	5	NULL	NULL	NULL	NULL	vivo screening	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The automated full time data collection of several different running parameters makes it also a suitable test for efficient in vivo screening of potential therapeutic compounds in this model for PD .
	manualset3
142608	5	408912	5	NULL	NULL	0	NULL	potential therapeutic compounds	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The automated full time data collection of several different running parameters makes it also a suitable test for efficient in vivo screening of potential therapeutic compounds in this model for PD .
	manualset3
142609	6	408912	5	NULL	NULL	0	NULL	model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The automated full time data collection of several different running parameters makes it also a suitable test for efficient in vivo screening of potential therapeutic compounds in this model for PD .
	manualset3
142610	7	408912	5	NULL	NULL	0	NULL	PD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The automated full time data collection of several different running parameters makes it also a suitable test for efficient in vivo screening of potential therapeutic compounds in this model for PD .
	manualset3
142611	1	408913	5	NULL	NULL	0	NULL	automated network	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The automated network automatically monitored the classification performance to determine when was the best time to stop training-after no improvement in the performance measure ( either highest correct classification rate , lowest mean squared error or highest log-sensitivity index value ) occurred in the subsequent 500 epochs .
	manualset3
142612	2	408913	5	NULL	NULL	0	NULL	classification performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The automated network automatically monitored the classification performance to determine when was the best time to stop training-after no improvement in the performance measure ( either highest correct classification rate , lowest mean squared error or highest log-sensitivity index value ) occurred in the subsequent 500 epochs .
	manualset3
142613	3	408913	5	NULL	NULL	0	NULL	 best time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The automated network automatically monitored the classification performance to determine when was the best time to stop training-after no improvement in the performance measure ( either highest correct classification rate , lowest mean squared error or highest log-sensitivity index value ) occurred in the subsequent 500 epochs .
	manualset3
142614	4	408913	5	NULL	NULL	0	NULL	training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The automated network automatically monitored the classification performance to determine when was the best time to stop training-after no improvement in the performance measure ( either highest correct classification rate , lowest mean squared error or highest log-sensitivity index value ) occurred in the subsequent 500 epochs .
	manualset3
142615	5	408913	5	NULL	NULL	0	NULL	improvement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The automated network automatically monitored the classification performance to determine when was the best time to stop training-after no improvement in the performance measure ( either highest correct classification rate , lowest mean squared error or highest log-sensitivity index value ) occurred in the subsequent 500 epochs .
	manualset3
142616	6	408913	5	NULL	NULL	NULL	NULL	performance measure	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The automated network automatically monitored the classification performance to determine when was the best time to stop training-after no improvement in the performance measure ( either highest correct classification rate , lowest mean squared error or highest log-sensitivity index value ) occurred in the subsequent 500 epochs .
	manualset3
142617	7	408913	5	NULL	NULL	0	NULL	highest correct classification rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The automated network automatically monitored the classification performance to determine when was the best time to stop training-after no improvement in the performance measure ( either highest correct classification rate , lowest mean squared error or highest log-sensitivity index value ) occurred in the subsequent 500 epochs .
	manualset3
142618	8	408913	5	NULL	NULL	0	NULL	lowest mean squared error	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The automated network automatically monitored the classification performance to determine when was the best time to stop training-after no improvement in the performance measure ( either highest correct classification rate , lowest mean squared error or highest log-sensitivity index value ) occurred in the subsequent 500 epochs .
	manualset3
142619	9	408913	5	NULL	NULL	0	NULL	highest log-sensitivity index value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The automated network automatically monitored the classification performance to determine when was the best time to stop training-after no improvement in the performance measure ( either highest correct classification rate , lowest mean squared error or highest log-sensitivity index value ) occurred in the subsequent 500 epochs .
	manualset3
142620	10	408913	5	NULL	NULL	0	NULL	500 epochs 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The automated network automatically monitored the classification performance to determine when was the best time to stop training-after no improvement in the performance measure ( either highest correct classification rate , lowest mean squared error or highest log-sensitivity index value ) occurred in the subsequent 500 epochs .
	manualset3
142621	1	408914	5	NULL	NULL	0	NULL	autopsy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The autopsy showed severe coronary artery atherosclerosis with remote and resolving myocardial microinfarcts , as well as the characteristic pink lividity of carbon monoxide poisoning , which was confirmed by laboratory analysis .
	manualset3
142622	2	408914	5	NULL	NULL	0	NULL	severe coronary artery atherosclerosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The autopsy showed severe coronary artery atherosclerosis with remote and resolving myocardial microinfarcts , as well as the characteristic pink lividity of carbon monoxide poisoning , which was confirmed by laboratory analysis .
	manualset3
142623	3	408914	5	NULL	NULL	0	NULL	myocardial microinfarcts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The autopsy showed severe coronary artery atherosclerosis with remote and resolving myocardial microinfarcts , as well as the characteristic pink lividity of carbon monoxide poisoning , which was confirmed by laboratory analysis .
	manualset3
142624	4	408914	5	NULL	NULL	0	NULL	 pink lividity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The autopsy showed severe coronary artery atherosclerosis with remote and resolving myocardial microinfarcts , as well as the characteristic pink lividity of carbon monoxide poisoning , which was confirmed by laboratory analysis .
	manualset3
142625	5	408914	5	NULL	NULL	0	NULL	carbon monoxide poisoning	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The autopsy showed severe coronary artery atherosclerosis with remote and resolving myocardial microinfarcts , as well as the characteristic pink lividity of carbon monoxide poisoning , which was confirmed by laboratory analysis .
	manualset3
142626	6	408914	5	NULL	NULL	0	NULL	laboratory analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The autopsy showed severe coronary artery atherosclerosis with remote and resolving myocardial microinfarcts , as well as the characteristic pink lividity of carbon monoxide poisoning , which was confirmed by laboratory analysis .
	manualset3
142627	1	408915	5	NULL	NULL	0	NULL	autoradiographic distribution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The autoradiographic distribution of 125I-Fe-transferrin receptors in rat brain has also been determined in vitro .
	manualset3
142628	2	408915	5	NULL	NULL	0	NULL	125I-Fe-transferrin receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The autoradiographic distribution of 125I-Fe-transferrin receptors in rat brain has also been determined in vitro .
	manualset3
142629	3	408915	5	NULL	NULL	0	NULL	rat brain 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The autoradiographic distribution of 125I-Fe-transferrin receptors in rat brain has also been determined in vitro .
	manualset3
142630	1	408916	5	NULL	NULL	0	NULL	availability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The availability of a xenogeneic species related to man similar as wolf to dog would markedly facilitate clinical xenotransplantation .
	manualset3
142631	2	408916	5	NULL	NULL	0	NULL	xenogeneic species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The availability of a xenogeneic species related to man similar as wolf to dog would markedly facilitate clinical xenotransplantation .
	manualset3
142632	3	408916	5	NULL	NULL	0	NULL	man 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The availability of a xenogeneic species related to man similar as wolf to dog would markedly facilitate clinical xenotransplantation .
	manualset3
142633	4	408916	5	NULL	NULL	0	NULL	wolf 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The availability of a xenogeneic species related to man similar as wolf to dog would markedly facilitate clinical xenotransplantation .
	manualset3
142634	5	408916	5	NULL	NULL	0	NULL	dog 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The availability of a xenogeneic species related to man similar as wolf to dog would markedly facilitate clinical xenotransplantation .
	manualset3
142635	6	408916	5	NULL	NULL	0	NULL	clinical xenotransplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The availability of a xenogeneic species related to man similar as wolf to dog would markedly facilitate clinical xenotransplantation .
	manualset3
142636	1	408917	5	NULL	NULL	0	NULL	availability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The availability of krypton-81m suitable for intravenous injection provides an easy means for assessing right ventricular function .
	manualset3
142637	2	408917	5	NULL	NULL	0	NULL	krypton-81m	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The availability of krypton-81m suitable for intravenous injection provides an easy means for assessing right ventricular function .
	manualset3
142638	3	408917	5	NULL	NULL	0	NULL	intravenous injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The availability of krypton-81m suitable for intravenous injection provides an easy means for assessing right ventricular function .
	manualset3
142639	4	408917	5	NULL	NULL	0	NULL	right ventricular function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The availability of krypton-81m suitable for intravenous injection provides an easy means for assessing right ventricular function .
	manualset3
142640	1	408918	5	NULL	NULL	0	NULL	evidence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The available evidence indicates , however , that S. mansoni is more prevalent in the country than is generally suspected .
	manualset3
142641	2	408918	5	NULL	NULL	0	NULL	S. mansoni	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The available evidence indicates , however , that S. mansoni is more prevalent in the country than is generally suspected .
	manualset3
142642	3	408918	5	NULL	NULL	0	NULL	country 	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The available evidence indicates , however , that S. mansoni is more prevalent in the country than is generally suspected .
	manualset3
142643	1	408919	5	NULL	NULL	0	NULL	available studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The available studies indicate that exposure to airborne particles is associated with hospital admissions for cardiovascular disease ; but the magnitude of this effect depends strongly on the specific disease category being considered , the time lag used in the analysis , and the type and amount of co-pollutants .
	manualset3
142644	2	408919	5	NULL	NULL	0	NULL	exposure 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The available studies indicate that exposure to airborne particles is associated with hospital admissions for cardiovascular disease ; but the magnitude of this effect depends strongly on the specific disease category being considered , the time lag used in the analysis , and the type and amount of co-pollutants .
	manualset3
142645	3	408919	5	NULL	NULL	0	NULL	airborne particles	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The available studies indicate that exposure to airborne particles is associated with hospital admissions for cardiovascular disease ; but the magnitude of this effect depends strongly on the specific disease category being considered , the time lag used in the analysis , and the type and amount of co-pollutants .
	manualset3
142646	4	408919	5	NULL	NULL	0	NULL	hospital admissions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The available studies indicate that exposure to airborne particles is associated with hospital admissions for cardiovascular disease ; but the magnitude of this effect depends strongly on the specific disease category being considered , the time lag used in the analysis , and the type and amount of co-pollutants .
	manualset3
142647	5	408919	5	NULL	NULL	0	NULL	cardiovascular disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The available studies indicate that exposure to airborne particles is associated with hospital admissions for cardiovascular disease ; but the magnitude of this effect depends strongly on the specific disease category being considered , the time lag used in the analysis , and the type and amount of co-pollutants .
	manualset3
142648	6	408919	5	NULL	NULL	0	NULL	magnitude 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The available studies indicate that exposure to airborne particles is associated with hospital admissions for cardiovascular disease ; but the magnitude of this effect depends strongly on the specific disease category being considered , the time lag used in the analysis , and the type and amount of co-pollutants .
	manualset3
142649	7	408919	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The available studies indicate that exposure to airborne particles is associated with hospital admissions for cardiovascular disease ; but the magnitude of this effect depends strongly on the specific disease category being considered , the time lag used in the analysis , and the type and amount of co-pollutants .
	manualset3
142650	8	408919	5	NULL	NULL	0	NULL	specific disease category	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The available studies indicate that exposure to airborne particles is associated with hospital admissions for cardiovascular disease ; but the magnitude of this effect depends strongly on the specific disease category being considered , the time lag used in the analysis , and the type and amount of co-pollutants .
	manualset3
142651	9	408919	5	NULL	NULL	0	NULL	time lag	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The available studies indicate that exposure to airborne particles is associated with hospital admissions for cardiovascular disease ; but the magnitude of this effect depends strongly on the specific disease category being considered , the time lag used in the analysis , and the type and amount of co-pollutants .
	manualset3
142652	10	408919	5	NULL	NULL	0	NULL	analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The available studies indicate that exposure to airborne particles is associated with hospital admissions for cardiovascular disease ; but the magnitude of this effect depends strongly on the specific disease category being considered , the time lag used in the analysis , and the type and amount of co-pollutants .
	manualset3
142653	11	408919	5	NULL	NULL	0	NULL	type 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The available studies indicate that exposure to airborne particles is associated with hospital admissions for cardiovascular disease ; but the magnitude of this effect depends strongly on the specific disease category being considered , the time lag used in the analysis , and the type and amount of co-pollutants .
	manualset3
142654	12	408919	5	NULL	NULL	0	NULL	amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The available studies indicate that exposure to airborne particles is associated with hospital admissions for cardiovascular disease ; but the magnitude of this effect depends strongly on the specific disease category being considered , the time lag used in the analysis , and the type and amount of co-pollutants .
	manualset3
142655	13	408919	5	NULL	NULL	0	NULL	co-pollutants	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The available studies indicate that exposure to airborne particles is associated with hospital admissions for cardiovascular disease ; but the magnitude of this effect depends strongly on the specific disease category being considered , the time lag used in the analysis , and the type and amount of co-pollutants .
	manualset3
142656	1	408920	5	NULL	NULL	0	NULL	average MPN/g ( SEM )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average MPN/g ( SEM ) was as follows : phosphate , 6.1910 ( 6 ) ( 2.4010 ( 6 ) ) ; hypophosphite , 2.6110 ( 6 ) ( 1.3510 ( 6 ) ) phosphite , 1.9110 ( 6 ) ( 1.0210 ( 6 ) ) ; aminoethylphosphonate , 3.9010 ( 6 ) ( 1.9510 ( 6 ) ) .
	manualset3
142657	2	408920	5	NULL	NULL	0	NULL	phosphate 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The average MPN/g ( SEM ) was as follows : phosphate , 6.1910 ( 6 ) ( 2.4010 ( 6 ) ) ; hypophosphite , 2.6110 ( 6 ) ( 1.3510 ( 6 ) ) phosphite , 1.9110 ( 6 ) ( 1.0210 ( 6 ) ) ; aminoethylphosphonate , 3.9010 ( 6 ) ( 1.9510 ( 6 ) ) .
	manualset3
142658	3	408920	5	NULL	NULL	0	NULL	6.1910 ( 6 ) ( 2.4010 ( 6 ) )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The average MPN/g ( SEM ) was as follows : phosphate , 6.1910 ( 6 ) ( 2.4010 ( 6 ) ) ; hypophosphite , 2.6110 ( 6 ) ( 1.3510 ( 6 ) ) phosphite , 1.9110 ( 6 ) ( 1.0210 ( 6 ) ) ; aminoethylphosphonate , 3.9010 ( 6 ) ( 1.9510 ( 6 ) ) .
	manualset3
142659	4	408920	5	NULL	NULL	0	NULL	hypophosphite 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The average MPN/g ( SEM ) was as follows : phosphate , 6.1910 ( 6 ) ( 2.4010 ( 6 ) ) ; hypophosphite , 2.6110 ( 6 ) ( 1.3510 ( 6 ) ) phosphite , 1.9110 ( 6 ) ( 1.0210 ( 6 ) ) ; aminoethylphosphonate , 3.9010 ( 6 ) ( 1.9510 ( 6 ) ) .
	manualset3
142660	5	408920	5	NULL	NULL	0	NULL	2.6110 ( 6 ) ( 1.3510 ( 6 ) )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The average MPN/g ( SEM ) was as follows : phosphate , 6.1910 ( 6 ) ( 2.4010 ( 6 ) ) ; hypophosphite , 2.6110 ( 6 ) ( 1.3510 ( 6 ) ) phosphite , 1.9110 ( 6 ) ( 1.0210 ( 6 ) ) ; aminoethylphosphonate , 3.9010 ( 6 ) ( 1.9510 ( 6 ) ) .
	manualset3
142661	6	408920	5	NULL	NULL	0	NULL	phosphite 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The average MPN/g ( SEM ) was as follows : phosphate , 6.1910 ( 6 ) ( 2.4010 ( 6 ) ) ; hypophosphite , 2.6110 ( 6 ) ( 1.3510 ( 6 ) ) phosphite , 1.9110 ( 6 ) ( 1.0210 ( 6 ) ) ; aminoethylphosphonate , 3.9010 ( 6 ) ( 1.9510 ( 6 ) ) .
	manualset3
142662	7	408920	5	NULL	NULL	0	NULL	1.9110 ( 6 ) ( 1.0210 ( 6 ) )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The average MPN/g ( SEM ) was as follows : phosphate , 6.1910 ( 6 ) ( 2.4010 ( 6 ) ) ; hypophosphite , 2.6110 ( 6 ) ( 1.3510 ( 6 ) ) phosphite , 1.9110 ( 6 ) ( 1.0210 ( 6 ) ) ; aminoethylphosphonate , 3.9010 ( 6 ) ( 1.9510 ( 6 ) ) .
	manualset3
142663	8	408920	5	NULL	NULL	0	NULL	aminoethylphosphonate 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The average MPN/g ( SEM ) was as follows : phosphate , 6.1910 ( 6 ) ( 2.4010 ( 6 ) ) ; hypophosphite , 2.6110 ( 6 ) ( 1.3510 ( 6 ) ) phosphite , 1.9110 ( 6 ) ( 1.0210 ( 6 ) ) ; aminoethylphosphonate , 3.9010 ( 6 ) ( 1.9510 ( 6 ) ) .
	manualset3
142664	9	408920	5	NULL	NULL	0	NULL	3.9010 ( 6 ) ( 1.9510 ( 6 ) )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The average MPN/g ( SEM ) was as follows : phosphate , 6.1910 ( 6 ) ( 2.4010 ( 6 ) ) ; hypophosphite , 2.6110 ( 6 ) ( 1.3510 ( 6 ) ) phosphite , 1.9110 ( 6 ) ( 1.0210 ( 6 ) ) ; aminoethylphosphonate , 3.9010 ( 6 ) ( 1.9510 ( 6 ) ) .
	manualset3
142665	1	408921	5	NULL	NULL	0	NULL	average correction	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average correction was 32 degrees ( 24 to 52 ) with a mean loss of correction after operation of 2.7 degrees ( 0 to 13 ) .
	manualset3
142666	2	408921	5	NULL	NULL	0	NULL	32 degrees ( 24 to 52 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The average correction was 32 degrees ( 24 to 52 ) with a mean loss of correction after operation of 2.7 degrees ( 0 to 13 ) .
	manualset3
142667	3	408921	5	NULL	NULL	0	NULL	mean loss of correction	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average correction was 32 degrees ( 24 to 52 ) with a mean loss of correction after operation of 2.7 degrees ( 0 to 13 ) .
	manualset3
142668	4	408921	5	NULL	NULL	0	NULL	operation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The average correction was 32 degrees ( 24 to 52 ) with a mean loss of correction after operation of 2.7 degrees ( 0 to 13 ) .
	manualset3
142669	5	408921	5	NULL	NULL	0	NULL	2.7 degrees ( 0 to 13 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The average correction was 32 degrees ( 24 to 52 ) with a mean loss of correction after operation of 2.7 degrees ( 0 to 13 ) .
	manualset3
142670	1	408922	5	NULL	NULL	0	NULL	average curve	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The average curve that can be plotted for the entire ensemble can be used as a solution to the problem , which is the main result of this study .
	manualset3
142671	2	408922	5	NULL	NULL	0	NULL	entire ensemble 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average curve that can be plotted for the entire ensemble can be used as a solution to the problem , which is the main result of this study .
	manualset3
142672	3	408922	5	NULL	NULL	0	NULL	solution 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average curve that can be plotted for the entire ensemble can be used as a solution to the problem , which is the main result of this study .
	manualset3
142673	4	408922	5	NULL	NULL	NULL	NULL	problem 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The average curve that can be plotted for the entire ensemble can be used as a solution to the problem , which is the main result of this study .
	manualset3
142674	5	408922	5	NULL	NULL	0	NULL	result 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The average curve that can be plotted for the entire ensemble can be used as a solution to the problem , which is the main result of this study .
	manualset3
142675	6	408922	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average curve that can be plotted for the entire ensemble can be used as a solution to the problem , which is the main result of this study .
	manualset3
142676	1	408923	5	NULL	NULL	0	NULL	average density	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average density of maxima is found to be & lt ; ( Z ) & gt ; = ( Z ) / Z ( c ) , where ( Z ) is a universal constant and Z ( c ) is the conductance autocorrelation length , which is system specific .
	manualset3
142677	2	408923	5	NULL	NULL	0	NULL	maxima 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average density of maxima is found to be & lt ; ( Z ) & gt ; = ( Z ) / Z ( c ) , where ( Z ) is a universal constant and Z ( c ) is the conductance autocorrelation length , which is system specific .
	manualset3
142678	3	408923	5	NULL	NULL	0	NULL	 & lt ; ( Z ) & gt ; = ( Z ) / Z ( c ) 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The average density of maxima is found to be & lt ; ( Z ) & gt ; = ( Z ) / Z ( c ) , where ( Z ) is a universal constant and Z ( c ) is the conductance autocorrelation length , which is system specific .
	manualset3
142679	4	408923	5	NULL	NULL	0	NULL	( Z ) 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The average density of maxima is found to be & lt ; ( Z ) & gt ; = ( Z ) / Z ( c ) , where ( Z ) is a universal constant and Z ( c ) is the conductance autocorrelation length , which is system specific .
	manualset3
142680	5	408923	5	NULL	NULL	0	NULL	universal constant 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average density of maxima is found to be & lt ; ( Z ) & gt ; = ( Z ) / Z ( c ) , where ( Z ) is a universal constant and Z ( c ) is the conductance autocorrelation length , which is system specific .
	manualset3
142681	6	408923	5	NULL	NULL	0	NULL	 Z ( c ) 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The average density of maxima is found to be & lt ; ( Z ) & gt ; = ( Z ) / Z ( c ) , where ( Z ) is a universal constant and Z ( c ) is the conductance autocorrelation length , which is system specific .
	manualset3
142682	7	408923	5	NULL	NULL	0	NULL	conductance autocorrelation length	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average density of maxima is found to be & lt ; ( Z ) & gt ; = ( Z ) / Z ( c ) , where ( Z ) is a universal constant and Z ( c ) is the conductance autocorrelation length , which is system specific .
	manualset3
142683	1	408924	5	NULL	NULL	0	NULL	average disease-free interval	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The average disease-free interval since primary treatment was significantly shorter in A with respect to S cases ( 40.3 vs. 28.5 months , P less than 0.001 ) as a consequence of the early detection achieved by CXR survey .
	manualset3
142684	2	408924	5	NULL	NULL	NULL	NULL	primary treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The average disease-free interval since primary treatment was significantly shorter in A with respect to S cases ( 40.3 vs. 28.5 months , P less than 0.001 ) as a consequence of the early detection achieved by CXR survey .
	manualset3
142685	3	408924	5	NULL	NULL	0	NULL	 A	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average disease-free interval since primary treatment was significantly shorter in A with respect to S cases ( 40.3 vs. 28.5 months , P less than 0.001 ) as a consequence of the early detection achieved by CXR survey .
	manualset3
142686	4	408924	5	NULL	NULL	NULL	NULL	 S cases	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The average disease-free interval since primary treatment was significantly shorter in A with respect to S cases ( 40.3 vs. 28.5 months , P less than 0.001 ) as a consequence of the early detection achieved by CXR survey .
	manualset3
142687	5	408924	5	NULL	NULL	0	NULL	 40.3 vs. 28.5 months 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The average disease-free interval since primary treatment was significantly shorter in A with respect to S cases ( 40.3 vs. 28.5 months , P less than 0.001 ) as a consequence of the early detection achieved by CXR survey .
	manualset3
142688	6	408924	5	NULL	NULL	0	NULL	P less than 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The average disease-free interval since primary treatment was significantly shorter in A with respect to S cases ( 40.3 vs. 28.5 months , P less than 0.001 ) as a consequence of the early detection achieved by CXR survey .
	manualset3
142689	7	408924	5	NULL	NULL	NULL	NULL	early detection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The average disease-free interval since primary treatment was significantly shorter in A with respect to S cases ( 40.3 vs. 28.5 months , P less than 0.001 ) as a consequence of the early detection achieved by CXR survey .
	manualset3
142690	8	408924	5	NULL	NULL	0	NULL	CXR survey	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The average disease-free interval since primary treatment was significantly shorter in A with respect to S cases ( 40.3 vs. 28.5 months , P less than 0.001 ) as a consequence of the early detection achieved by CXR survey .
	manualset3
142691	1	408925	5	NULL	NULL	0	NULL	self-administered evaluation questionnaire 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A self-administered evaluation questionnaire was completed by 672 adolescents aged 12-18 years the Dutch equivalent of the 8th and 10th grade of secondary education .
	manualset3
142692	2	408925	5	NULL	NULL	0	NULL	672 adolescents	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A self-administered evaluation questionnaire was completed by 672 adolescents aged 12-18 years the Dutch equivalent of the 8th and 10th grade of secondary education .
	manualset3
142693	3	408925	5	NULL	NULL	0	NULL	12-18 years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A self-administered evaluation questionnaire was completed by 672 adolescents aged 12-18 years the Dutch equivalent of the 8th and 10th grade of secondary education .
	manualset3
142694	4	408925	5	NULL	NULL	0	NULL	Dutch equivalent	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A self-administered evaluation questionnaire was completed by 672 adolescents aged 12-18 years the Dutch equivalent of the 8th and 10th grade of secondary education .
	manualset3
142695	5	408925	5	NULL	NULL	0	NULL	8th grade	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A self-administered evaluation questionnaire was completed by 672 adolescents aged 12-18 years the Dutch equivalent of the 8th and 10th grade of secondary education .
	manualset3
142696	6	408925	5	NULL	NULL	0	NULL	10th grade 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A self-administered evaluation questionnaire was completed by 672 adolescents aged 12-18 years the Dutch equivalent of the 8th and 10th grade of secondary education .
	manualset3
142697	7	408925	5	NULL	NULL	0	NULL	secondary education	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A self-administered evaluation questionnaire was completed by 672 adolescents aged 12-18 years the Dutch equivalent of the 8th and 10th grade of secondary education .
	manualset3
142698	1	408926	5	NULL	NULL	0	NULL	average minimal lethal intraperitoneal dose 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average minimal lethal intraperitoneal dose of the toxin in mice was approximately 10 ( 6 ) per ml .
	manualset3
142699	2	408926	5	NULL	NULL	0	NULL	toxin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The average minimal lethal intraperitoneal dose of the toxin in mice was approximately 10 ( 6 ) per ml .
	manualset3
142700	3	408926	5	NULL	NULL	0	NULL	mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The average minimal lethal intraperitoneal dose of the toxin in mice was approximately 10 ( 6 ) per ml .
	manualset3
142701	4	408926	5	NULL	NULL	0	NULL	 10 ( 6 ) per ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The average minimal lethal intraperitoneal dose of the toxin in mice was approximately 10 ( 6 ) per ml .
	manualset3
142702	1	408927	5	NULL	NULL	0	NULL	average number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average number of operations performed with processing control was established along with the total cost per minute of labor expended .
	manualset3
142703	2	408927	5	NULL	NULL	0	NULL	operations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The average number of operations performed with processing control was established along with the total cost per minute of labor expended .
	manualset3
142704	3	408927	5	NULL	NULL	0	NULL	processing control 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average number of operations performed with processing control was established along with the total cost per minute of labor expended .
	manualset3
142705	4	408927	5	NULL	NULL	0	NULL	total cost per minute	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average number of operations performed with processing control was established along with the total cost per minute of labor expended .
	manualset3
142706	5	408927	5	NULL	NULL	0	NULL	labor 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average number of operations performed with processing control was established along with the total cost per minute of labor expended .
	manualset3
142707	1	408928	5	NULL	NULL	0	NULL	average onset times	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average onset times of rocuronium ( 172 s ) and vecuronium ( 192 s ) were significantly shorter than that of mivacurium ( 229 s ) .
	manualset3
142708	2	408928	5	NULL	NULL	0	NULL	rocuronium 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The average onset times of rocuronium ( 172 s ) and vecuronium ( 192 s ) were significantly shorter than that of mivacurium ( 229 s ) .
	manualset3
142709	3	408928	5	NULL	NULL	0	NULL	172 s	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The average onset times of rocuronium ( 172 s ) and vecuronium ( 192 s ) were significantly shorter than that of mivacurium ( 229 s ) .
	manualset3
142710	4	408928	5	NULL	NULL	0	NULL	vecuronium 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The average onset times of rocuronium ( 172 s ) and vecuronium ( 192 s ) were significantly shorter than that of mivacurium ( 229 s ) .
	manualset3
142711	5	408928	5	NULL	NULL	0	NULL	192 s	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The average onset times of rocuronium ( 172 s ) and vecuronium ( 192 s ) were significantly shorter than that of mivacurium ( 229 s ) .
	manualset3
142712	6	408928	5	NULL	NULL	0	NULL	mivacurium 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The average onset times of rocuronium ( 172 s ) and vecuronium ( 192 s ) were significantly shorter than that of mivacurium ( 229 s ) .
	manualset3
142713	7	408928	5	NULL	NULL	0	NULL	229 s	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The average onset times of rocuronium ( 172 s ) and vecuronium ( 192 s ) were significantly shorter than that of mivacurium ( 229 s ) .
	manualset3
142714	1	408929	5	NULL	NULL	0	NULL	average quantity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average quantity of training in the final intervention group ( n = 19 ) was 29.9 floors/workday or 36 , 790 kpm/week and in the control group 4.6 and 5980 correspondingly .
	manualset3
142715	2	408929	5	NULL	NULL	0	NULL	training 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The average quantity of training in the final intervention group ( n = 19 ) was 29.9 floors/workday or 36 , 790 kpm/week and in the control group 4.6 and 5980 correspondingly .
	manualset3
142716	3	408929	5	NULL	NULL	0	NULL	final intervention group	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average quantity of training in the final intervention group ( n = 19 ) was 29.9 floors/workday or 36 , 790 kpm/week and in the control group 4.6 and 5980 correspondingly .
	manualset3
142717	4	408929	5	NULL	NULL	0	NULL	 n = 19 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The average quantity of training in the final intervention group ( n = 19 ) was 29.9 floors/workday or 36 , 790 kpm/week and in the control group 4.6 and 5980 correspondingly .
	manualset3
142718	5	408929	5	NULL	NULL	0	NULL	29.9 floors/workday 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The average quantity of training in the final intervention group ( n = 19 ) was 29.9 floors/workday or 36 , 790 kpm/week and in the control group 4.6 and 5980 correspondingly .
	manualset3
142719	6	408929	5	NULL	NULL	0	NULL	36 , 790 kpm/week	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The average quantity of training in the final intervention group ( n = 19 ) was 29.9 floors/workday or 36 , 790 kpm/week and in the control group 4.6 and 5980 correspondingly .
	manualset3
142720	7	408929	5	NULL	NULL	0	NULL	control group 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average quantity of training in the final intervention group ( n = 19 ) was 29.9 floors/workday or 36 , 790 kpm/week and in the control group 4.6 and 5980 correspondingly .
	manualset3
142721	8	408929	5	NULL	NULL	0	NULL	4.6 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The average quantity of training in the final intervention group ( n = 19 ) was 29.9 floors/workday or 36 , 790 kpm/week and in the control group 4.6 and 5980 correspondingly .
	manualset3
142722	9	408929	5	NULL	NULL	0	NULL	5980 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The average quantity of training in the final intervention group ( n = 19 ) was 29.9 floors/workday or 36 , 790 kpm/week and in the control group 4.6 and 5980 correspondingly .
	manualset3
142723	1	408930	5	NULL	NULL	0	NULL	axial positions	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The axial positions are occupied by two bridging diaminobutane molecules ( Cu-N = 2.011 ( 4 ) A ) that connect the Cu atoms into chains parallel to the above plane .
	manualset3
142724	2	408930	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The axial positions are occupied by two bridging diaminobutane molecules ( Cu-N = 2.011 ( 4 ) A ) that connect the Cu atoms into chains parallel to the above plane .
	manualset3
142725	3	408930	5	NULL	NULL	NULL	NULL	diaminobutane molecules	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The axial positions are occupied by two bridging diaminobutane molecules ( Cu-N = 2.011 ( 4 ) A ) that connect the Cu atoms into chains parallel to the above plane .
	manualset3
142726	4	408930	5	NULL	NULL	0	NULL	Cu-N = 2.011 ( 4 ) A	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The axial positions are occupied by two bridging diaminobutane molecules ( Cu-N = 2.011 ( 4 ) A ) that connect the Cu atoms into chains parallel to the above plane .
	manualset3
142727	5	408930	5	NULL	NULL	0	NULL	Cu atoms	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The axial positions are occupied by two bridging diaminobutane molecules ( Cu-N = 2.011 ( 4 ) A ) that connect the Cu atoms into chains parallel to the above plane .
	manualset3
142728	6	408930	5	NULL	NULL	0	NULL	chains 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The axial positions are occupied by two bridging diaminobutane molecules ( Cu-N = 2.011 ( 4 ) A ) that connect the Cu atoms into chains parallel to the above plane .
	manualset3
142729	7	408930	5	NULL	NULL	0	NULL	plane 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The axial positions are occupied by two bridging diaminobutane molecules ( Cu-N = 2.011 ( 4 ) A ) that connect the Cu atoms into chains parallel to the above plane .
	manualset3
142730	1	408931	5	NULL	NULL	0	NULL	self-directed adherence management program 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A self-directed adherence management program for patients with heart failure completing combined aerobic and resistance exercise training .
	manualset3
142731	2	408931	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A self-directed adherence management program for patients with heart failure completing combined aerobic and resistance exercise training .
	manualset3
142732	3	408931	5	NULL	NULL	0	NULL	heart failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A self-directed adherence management program for patients with heart failure completing combined aerobic and resistance exercise training .
	manualset3
142733	4	408931	5	NULL	NULL	NULL	NULL	combined aerobic and resistance exercise training	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A self-directed adherence management program for patients with heart failure completing combined aerobic and resistance exercise training .
	manualset3
142734	1	408932	5	NULL	NULL	0	NULL	bacteria 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacteria tested showed great differences in sensitivity to polyphosphoric acid , but synergism with enterocin AS-48 was confirmed in all cases .
	manualset3
142735	2	408932	5	NULL	NULL	NULL	NULL	differences 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The bacteria tested showed great differences in sensitivity to polyphosphoric acid , but synergism with enterocin AS-48 was confirmed in all cases .
	manualset3
142736	3	408932	5	NULL	NULL	0	NULL	sensitivity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacteria tested showed great differences in sensitivity to polyphosphoric acid , but synergism with enterocin AS-48 was confirmed in all cases .
	manualset3
142737	4	408932	5	NULL	NULL	0	NULL	polyphosphoric acid	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacteria tested showed great differences in sensitivity to polyphosphoric acid , but synergism with enterocin AS-48 was confirmed in all cases .
	manualset3
142738	5	408932	5	NULL	NULL	0	NULL	synergism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacteria tested showed great differences in sensitivity to polyphosphoric acid , but synergism with enterocin AS-48 was confirmed in all cases .
	manualset3
142739	6	408932	5	NULL	NULL	0	NULL	enterocin AS-48	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacteria tested showed great differences in sensitivity to polyphosphoric acid , but synergism with enterocin AS-48 was confirmed in all cases .
	manualset3
142740	7	408932	5	NULL	NULL	0	NULL	cases 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacteria tested showed great differences in sensitivity to polyphosphoric acid , but synergism with enterocin AS-48 was confirmed in all cases .
	manualset3
142741	1	408933	5	NULL	NULL	0	NULL	bacterial isolates 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacterial isolates in the 13 patients were more suggestive of reactivated chronic infection than catheter associated UTI .
	manualset3
142742	2	408933	5	NULL	NULL	0	NULL	 13 patients	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacterial isolates in the 13 patients were more suggestive of reactivated chronic infection than catheter associated UTI .
	manualset3
142743	3	408933	5	NULL	NULL	0	NULL	reactivated chronic infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacterial isolates in the 13 patients were more suggestive of reactivated chronic infection than catheter associated UTI .
	manualset3
142744	4	408933	5	NULL	NULL	0	NULL	catheter associated UTI 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacterial isolates in the 13 patients were more suggestive of reactivated chronic infection than catheter associated UTI .
	manualset3
142745	1	408934	5	NULL	NULL	0	NULL	bacterial population	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacterial population is now similar to that observed in other European countries .
	manualset3
142746	2	408934	5	NULL	NULL	0	NULL	other European countries	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacterial population is now similar to that observed in other European countries .
	manualset3
142747	1	408935	5	NULL	NULL	NULL	NULL	bacteriologic yield 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The bacteriologic yield was 62 % ( 52/84 ) for the pleural tissue , 12 % ( 10/84 ) for pleural fluid , and 52 % ( 44/84 ) for sputum cultures obtained by SI .
	manualset3
142748	2	408935	5	NULL	NULL	0	NULL	 62 % ( 52/84 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacteriologic yield was 62 % ( 52/84 ) for the pleural tissue , 12 % ( 10/84 ) for pleural fluid , and 52 % ( 44/84 ) for sputum cultures obtained by SI .
	manualset3
142749	3	408935	5	NULL	NULL	0	NULL	pleural tissue 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacteriologic yield was 62 % ( 52/84 ) for the pleural tissue , 12 % ( 10/84 ) for pleural fluid , and 52 % ( 44/84 ) for sputum cultures obtained by SI .
	manualset3
142750	4	408935	5	NULL	NULL	0	NULL	12 % ( 10/84 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacteriologic yield was 62 % ( 52/84 ) for the pleural tissue , 12 % ( 10/84 ) for pleural fluid , and 52 % ( 44/84 ) for sputum cultures obtained by SI .
	manualset3
142751	5	408935	5	NULL	NULL	0	NULL	pleural fluid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacteriologic yield was 62 % ( 52/84 ) for the pleural tissue , 12 % ( 10/84 ) for pleural fluid , and 52 % ( 44/84 ) for sputum cultures obtained by SI .
	manualset3
142752	6	408935	5	NULL	NULL	0	NULL	52 % ( 44/84 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacteriologic yield was 62 % ( 52/84 ) for the pleural tissue , 12 % ( 10/84 ) for pleural fluid , and 52 % ( 44/84 ) for sputum cultures obtained by SI .
	manualset3
142753	7	408935	5	NULL	NULL	NULL	NULL	sputum cultures 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The bacteriologic yield was 62 % ( 52/84 ) for the pleural tissue , 12 % ( 10/84 ) for pleural fluid , and 52 % ( 44/84 ) for sputum cultures obtained by SI .
	manualset3
142754	8	408935	5	NULL	NULL	0	NULL	SI 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacteriologic yield was 62 % ( 52/84 ) for the pleural tissue , 12 % ( 10/84 ) for pleural fluid , and 52 % ( 44/84 ) for sputum cultures obtained by SI .
	manualset3
142755	1	408936	5	NULL	NULL	0	NULL	bacteriological examination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacteriological examination of bronchial secretion in various lung diseases showed a prevailing growth by diplococcus pneumoniae , and more sterile conditions in the peripheral bronchial airways of 56 patients .
	manualset3
142756	2	408936	5	NULL	NULL	0	NULL	bronchial secretion	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacteriological examination of bronchial secretion in various lung diseases showed a prevailing growth by diplococcus pneumoniae , and more sterile conditions in the peripheral bronchial airways of 56 patients .
	manualset3
142757	3	408936	5	NULL	NULL	0	NULL	lung diseases 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacteriological examination of bronchial secretion in various lung diseases showed a prevailing growth by diplococcus pneumoniae , and more sterile conditions in the peripheral bronchial airways of 56 patients .
	manualset3
142758	4	408936	5	NULL	NULL	0	NULL	prevailing growth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacteriological examination of bronchial secretion in various lung diseases showed a prevailing growth by diplococcus pneumoniae , and more sterile conditions in the peripheral bronchial airways of 56 patients .
	manualset3
142759	5	408936	5	NULL	NULL	0	NULL	diplococcus pneumoniae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacteriological examination of bronchial secretion in various lung diseases showed a prevailing growth by diplococcus pneumoniae , and more sterile conditions in the peripheral bronchial airways of 56 patients .
	manualset3
142760	6	408936	5	NULL	NULL	0	NULL	sterile conditions 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacteriological examination of bronchial secretion in various lung diseases showed a prevailing growth by diplococcus pneumoniae , and more sterile conditions in the peripheral bronchial airways of 56 patients .
	manualset3
142761	7	408936	5	NULL	NULL	0	NULL	peripheral bronchial airways	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacteriological examination of bronchial secretion in various lung diseases showed a prevailing growth by diplococcus pneumoniae , and more sterile conditions in the peripheral bronchial airways of 56 patients .
	manualset3
142762	8	408936	5	NULL	NULL	0	NULL	 56 patients	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacteriological examination of bronchial secretion in various lung diseases showed a prevailing growth by diplococcus pneumoniae , and more sterile conditions in the peripheral bronchial airways of 56 patients .
	manualset3
142763	1	408937	5	NULL	NULL	0	NULL	bacterium 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacterium showed the peptidoglycan type Lys-Ala3 ( variation A3alpha ) , MK-7 ( H2 ) was the major menaquinone and anteiso-C ( 15 : 0 ) and anteiso-C ( 17 : 0 ) were the major fatty acids .
	manualset3
142764	2	408937	5	NULL	NULL	0	NULL	peptidoglycan type Lys-Ala3 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacterium showed the peptidoglycan type Lys-Ala3 ( variation A3alpha ) , MK-7 ( H2 ) was the major menaquinone and anteiso-C ( 15 : 0 ) and anteiso-C ( 17 : 0 ) were the major fatty acids .
	manualset3
142765	3	408937	5	NULL	NULL	0	NULL	variation A3alpha	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacterium showed the peptidoglycan type Lys-Ala3 ( variation A3alpha ) , MK-7 ( H2 ) was the major menaquinone and anteiso-C ( 15 : 0 ) and anteiso-C ( 17 : 0 ) were the major fatty acids .
	manualset3
142766	4	408937	5	NULL	NULL	0	NULL	MK-7 ( H2 )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacterium showed the peptidoglycan type Lys-Ala3 ( variation A3alpha ) , MK-7 ( H2 ) was the major menaquinone and anteiso-C ( 15 : 0 ) and anteiso-C ( 17 : 0 ) were the major fatty acids .
	manualset3
142767	5	408937	5	NULL	NULL	0	NULL	menaquinone 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacterium showed the peptidoglycan type Lys-Ala3 ( variation A3alpha ) , MK-7 ( H2 ) was the major menaquinone and anteiso-C ( 15 : 0 ) and anteiso-C ( 17 : 0 ) were the major fatty acids .
	manualset3
142768	6	408937	5	NULL	NULL	0	NULL	anteiso-C ( 15 : 0 ) 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacterium showed the peptidoglycan type Lys-Ala3 ( variation A3alpha ) , MK-7 ( H2 ) was the major menaquinone and anteiso-C ( 15 : 0 ) and anteiso-C ( 17 : 0 ) were the major fatty acids .
	manualset3
142769	7	408937	5	NULL	NULL	0	NULL	anteiso-C ( 17 : 0 )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacterium showed the peptidoglycan type Lys-Ala3 ( variation A3alpha ) , MK-7 ( H2 ) was the major menaquinone and anteiso-C ( 15 : 0 ) and anteiso-C ( 17 : 0 ) were the major fatty acids .
	manualset3
142770	8	408937	5	NULL	NULL	0	NULL	fatty acids	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The bacterium showed the peptidoglycan type Lys-Ala3 ( variation A3alpha ) , MK-7 ( H2 ) was the major menaquinone and anteiso-C ( 15 : 0 ) and anteiso-C ( 17 : 0 ) were the major fatty acids .
	manualset3
142771	1	408938	5	NULL	NULL	0	NULL	band gap value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The band gap value is distinctly different from those calculated previously for the M-IRMOF-1 ( benzene-1 , 4 - dicarboxylate linker ; ca .
	manualset3
142772	2	408938	5	NULL	NULL	0	NULL	M-IRMOF-1	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The band gap value is distinctly different from those calculated previously for the M-IRMOF-1 ( benzene-1 , 4 - dicarboxylate linker ; ca .
	manualset3
142773	3	408938	5	NULL	NULL	0	NULL	benzene-1 , 4 - dicarboxylate linker	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The band gap value is distinctly different from those calculated previously for the M-IRMOF-1 ( benzene-1 , 4 - dicarboxylate linker ; ca .
	manualset3
142774	4	408938	5	NULL	NULL	0	NULL	ca 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The band gap value is distinctly different from those calculated previously for the M-IRMOF-1 ( benzene-1 , 4 - dicarboxylate linker ; ca .
	manualset3
142775	1	408939	5	NULL	NULL	0	NULL	baroreflex sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The baroreflex sensitivity and the baroreflex effectiveness index were reduced by 36 % and 64 % , respectively ( P & lt ; 0.01 for both ) in patients five weeks after coronary artery bypass grafting compared to healthy subjects ( HS ) .
	manualset3
142776	2	408939	5	NULL	NULL	0	NULL	baroreflex effectiveness index 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The baroreflex sensitivity and the baroreflex effectiveness index were reduced by 36 % and 64 % , respectively ( P & lt ; 0.01 for both ) in patients five weeks after coronary artery bypass grafting compared to healthy subjects ( HS ) .
	manualset3
142777	3	408939	5	NULL	NULL	0	NULL	 36 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The baroreflex sensitivity and the baroreflex effectiveness index were reduced by 36 % and 64 % , respectively ( P & lt ; 0.01 for both ) in patients five weeks after coronary artery bypass grafting compared to healthy subjects ( HS ) .
	manualset3
142778	4	408939	5	NULL	NULL	0	NULL	 64 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The baroreflex sensitivity and the baroreflex effectiveness index were reduced by 36 % and 64 % , respectively ( P & lt ; 0.01 for both ) in patients five weeks after coronary artery bypass grafting compared to healthy subjects ( HS ) .
	manualset3
142779	5	408939	5	NULL	NULL	0	NULL	P & lt ; 0.01 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The baroreflex sensitivity and the baroreflex effectiveness index were reduced by 36 % and 64 % , respectively ( P & lt ; 0.01 for both ) in patients five weeks after coronary artery bypass grafting compared to healthy subjects ( HS ) .
	manualset3
142780	6	408939	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The baroreflex sensitivity and the baroreflex effectiveness index were reduced by 36 % and 64 % , respectively ( P & lt ; 0.01 for both ) in patients five weeks after coronary artery bypass grafting compared to healthy subjects ( HS ) .
	manualset3
142781	7	408939	5	NULL	NULL	0	NULL	five weeks	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The baroreflex sensitivity and the baroreflex effectiveness index were reduced by 36 % and 64 % , respectively ( P & lt ; 0.01 for both ) in patients five weeks after coronary artery bypass grafting compared to healthy subjects ( HS ) .
	manualset3
142782	8	408939	5	NULL	NULL	0	NULL	coronary artery bypass grafting 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The baroreflex sensitivity and the baroreflex effectiveness index were reduced by 36 % and 64 % , respectively ( P & lt ; 0.01 for both ) in patients five weeks after coronary artery bypass grafting compared to healthy subjects ( HS ) .
	manualset3
142783	9	408939	5	NULL	NULL	0	NULL	healthy subjects ( HS )	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The baroreflex sensitivity and the baroreflex effectiveness index were reduced by 36 % and 64 % , respectively ( P & lt ; 0.01 for both ) in patients five weeks after coronary artery bypass grafting compared to healthy subjects ( HS ) .
	manualset3
142784	1	408940	5	NULL	NULL	0	NULL	barrier properties 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The barrier properties of layer-by-layer polyelectrolyte films ( PE ) composed of polyacrylic acid and polyallylamine hydro-chloride layers on Ag-surfaces were compared between untreated , thermally crosslinked , and Ag-nanoparticles containing samples .
	manualset3
142785	2	408940	5	NULL	NULL	0	NULL	layer-by-layer polyelectrolyte films ( PE )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The barrier properties of layer-by-layer polyelectrolyte films ( PE ) composed of polyacrylic acid and polyallylamine hydro-chloride layers on Ag-surfaces were compared between untreated , thermally crosslinked , and Ag-nanoparticles containing samples .
	manualset3
142786	3	408940	5	NULL	NULL	0	NULL	polyacrylic acid	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The barrier properties of layer-by-layer polyelectrolyte films ( PE ) composed of polyacrylic acid and polyallylamine hydro-chloride layers on Ag-surfaces were compared between untreated , thermally crosslinked , and Ag-nanoparticles containing samples .
	manualset3
142787	4	408940	5	NULL	NULL	0	NULL	polyallylamine hydro-chloride layers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The barrier properties of layer-by-layer polyelectrolyte films ( PE ) composed of polyacrylic acid and polyallylamine hydro-chloride layers on Ag-surfaces were compared between untreated , thermally crosslinked , and Ag-nanoparticles containing samples .
	manualset3
142788	5	408940	5	NULL	NULL	0	NULL	Ag-surfaces	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The barrier properties of layer-by-layer polyelectrolyte films ( PE ) composed of polyacrylic acid and polyallylamine hydro-chloride layers on Ag-surfaces were compared between untreated , thermally crosslinked , and Ag-nanoparticles containing samples .
	manualset3
142789	6	408940	5	NULL	NULL	0	NULL	Ag-nanoparticles	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The barrier properties of layer-by-layer polyelectrolyte films ( PE ) composed of polyacrylic acid and polyallylamine hydro-chloride layers on Ag-surfaces were compared between untreated , thermally crosslinked , and Ag-nanoparticles containing samples .
	manualset3
142790	7	408940	5	NULL	NULL	0	NULL	samples 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The barrier properties of layer-by-layer polyelectrolyte films ( PE ) composed of polyacrylic acid and polyallylamine hydro-chloride layers on Ag-surfaces were compared between untreated , thermally crosslinked , and Ag-nanoparticles containing samples .
	manualset3
142791	1	408941	5	NULL	NULL	0	NULL	barrier properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The barrier properties of this endothelial surface layer are deduced from the rate of tracer penetration into the layer and the mechanics of red and white cell movement through capillary microvessels .
	manualset3
142792	2	408941	5	NULL	NULL	NULL	NULL	endothelial surface layer	AnatomicalPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The barrier properties of this endothelial surface layer are deduced from the rate of tracer penetration into the layer and the mechanics of red and white cell movement through capillary microvessels .
	manualset3
142793	3	408941	5	NULL	NULL	0	NULL	rate of tracer penetration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The barrier properties of this endothelial surface layer are deduced from the rate of tracer penetration into the layer and the mechanics of red and white cell movement through capillary microvessels .
	manualset3
142794	4	408941	5	NULL	NULL	NULL	NULL	layer 	AnatomicalPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The barrier properties of this endothelial surface layer are deduced from the rate of tracer penetration into the layer and the mechanics of red and white cell movement through capillary microvessels .
	manualset3
142795	5	408941	5	NULL	NULL	0	NULL	mechanics 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The barrier properties of this endothelial surface layer are deduced from the rate of tracer penetration into the layer and the mechanics of red and white cell movement through capillary microvessels .
	manualset3
142796	6	408941	5	NULL	NULL	0	NULL	red cell movement	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The barrier properties of this endothelial surface layer are deduced from the rate of tracer penetration into the layer and the mechanics of red and white cell movement through capillary microvessels .
	manualset3
142797	7	408941	5	NULL	NULL	0	NULL	white cell movement	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The barrier properties of this endothelial surface layer are deduced from the rate of tracer penetration into the layer and the mechanics of red and white cell movement through capillary microvessels .
	manualset3
142798	8	408941	5	NULL	NULL	0	NULL	capillary microvessels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The barrier properties of this endothelial surface layer are deduced from the rate of tracer penetration into the layer and the mechanics of red and white cell movement through capillary microvessels .
	manualset3
142799	1	408942	5	NULL	NULL	0	NULL	base compositions 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The base compositions proximal to the 5 ' ends of mRNA 's from promoters on these DNA fragments were elucidated by the polymerase initiation assay , in which the addition of various combinations of nucleoside triphosphates to the reaction allowed RNA polymerase to form high-salt-resistant initiation complexes with some of the known SmaI + EcoRI , EcoRI + HindIII , or HaeIII restriction fragments of lambda rifd 18 DNA .
	manualset3
142800	2	408942	5	NULL	NULL	0	NULL	5 ' ends of mRNA 's	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The base compositions proximal to the 5 ' ends of mRNA 's from promoters on these DNA fragments were elucidated by the polymerase initiation assay , in which the addition of various combinations of nucleoside triphosphates to the reaction allowed RNA polymerase to form high-salt-resistant initiation complexes with some of the known SmaI + EcoRI , EcoRI + HindIII , or HaeIII restriction fragments of lambda rifd 18 DNA .
	manualset3
142801	3	408942	5	NULL	NULL	0	NULL	promoters 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The base compositions proximal to the 5 ' ends of mRNA 's from promoters on these DNA fragments were elucidated by the polymerase initiation assay , in which the addition of various combinations of nucleoside triphosphates to the reaction allowed RNA polymerase to form high-salt-resistant initiation complexes with some of the known SmaI + EcoRI , EcoRI + HindIII , or HaeIII restriction fragments of lambda rifd 18 DNA .
	manualset3
142802	4	408942	5	NULL	NULL	0	NULL	DNA fragments	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The base compositions proximal to the 5 ' ends of mRNA 's from promoters on these DNA fragments were elucidated by the polymerase initiation assay , in which the addition of various combinations of nucleoside triphosphates to the reaction allowed RNA polymerase to form high-salt-resistant initiation complexes with some of the known SmaI + EcoRI , EcoRI + HindIII , or HaeIII restriction fragments of lambda rifd 18 DNA .
	manualset3
142803	5	408942	5	NULL	NULL	0	NULL	polymerase initiation assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The base compositions proximal to the 5 ' ends of mRNA 's from promoters on these DNA fragments were elucidated by the polymerase initiation assay , in which the addition of various combinations of nucleoside triphosphates to the reaction allowed RNA polymerase to form high-salt-resistant initiation complexes with some of the known SmaI + EcoRI , EcoRI + HindIII , or HaeIII restriction fragments of lambda rifd 18 DNA .
	manualset3
142804	6	408942	5	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The base compositions proximal to the 5 ' ends of mRNA 's from promoters on these DNA fragments were elucidated by the polymerase initiation assay , in which the addition of various combinations of nucleoside triphosphates to the reaction allowed RNA polymerase to form high-salt-resistant initiation complexes with some of the known SmaI + EcoRI , EcoRI + HindIII , or HaeIII restriction fragments of lambda rifd 18 DNA .
	manualset3
142805	7	408942	5	NULL	NULL	0	NULL	combinations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The base compositions proximal to the 5 ' ends of mRNA 's from promoters on these DNA fragments were elucidated by the polymerase initiation assay , in which the addition of various combinations of nucleoside triphosphates to the reaction allowed RNA polymerase to form high-salt-resistant initiation complexes with some of the known SmaI + EcoRI , EcoRI + HindIII , or HaeIII restriction fragments of lambda rifd 18 DNA .
	manualset3
142806	8	408942	5	NULL	NULL	0	NULL	nucleoside triphosphates	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The base compositions proximal to the 5 ' ends of mRNA 's from promoters on these DNA fragments were elucidated by the polymerase initiation assay , in which the addition of various combinations of nucleoside triphosphates to the reaction allowed RNA polymerase to form high-salt-resistant initiation complexes with some of the known SmaI + EcoRI , EcoRI + HindIII , or HaeIII restriction fragments of lambda rifd 18 DNA .
	manualset3
142807	9	408942	5	NULL	NULL	0	NULL	reaction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The base compositions proximal to the 5 ' ends of mRNA 's from promoters on these DNA fragments were elucidated by the polymerase initiation assay , in which the addition of various combinations of nucleoside triphosphates to the reaction allowed RNA polymerase to form high-salt-resistant initiation complexes with some of the known SmaI + EcoRI , EcoRI + HindIII , or HaeIII restriction fragments of lambda rifd 18 DNA .
	manualset3
142808	10	408942	5	NULL	NULL	0	NULL	RNA polymerase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The base compositions proximal to the 5 ' ends of mRNA 's from promoters on these DNA fragments were elucidated by the polymerase initiation assay , in which the addition of various combinations of nucleoside triphosphates to the reaction allowed RNA polymerase to form high-salt-resistant initiation complexes with some of the known SmaI + EcoRI , EcoRI + HindIII , or HaeIII restriction fragments of lambda rifd 18 DNA .
	manualset3
142809	11	408942	5	NULL	NULL	0	NULL	high-salt-resistant initiation complexes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The base compositions proximal to the 5 ' ends of mRNA 's from promoters on these DNA fragments were elucidated by the polymerase initiation assay , in which the addition of various combinations of nucleoside triphosphates to the reaction allowed RNA polymerase to form high-salt-resistant initiation complexes with some of the known SmaI + EcoRI , EcoRI + HindIII , or HaeIII restriction fragments of lambda rifd 18 DNA .
	manualset3
142810	12	408942	5	NULL	NULL	0	NULL	SmaI + EcoRI 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The base compositions proximal to the 5 ' ends of mRNA 's from promoters on these DNA fragments were elucidated by the polymerase initiation assay , in which the addition of various combinations of nucleoside triphosphates to the reaction allowed RNA polymerase to form high-salt-resistant initiation complexes with some of the known SmaI + EcoRI , EcoRI + HindIII , or HaeIII restriction fragments of lambda rifd 18 DNA .
	manualset3
142811	13	408942	5	NULL	NULL	0	NULL	EcoRI + HindIII	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The base compositions proximal to the 5 ' ends of mRNA 's from promoters on these DNA fragments were elucidated by the polymerase initiation assay , in which the addition of various combinations of nucleoside triphosphates to the reaction allowed RNA polymerase to form high-salt-resistant initiation complexes with some of the known SmaI + EcoRI , EcoRI + HindIII , or HaeIII restriction fragments of lambda rifd 18 DNA .
	manualset3
142812	14	408942	5	NULL	NULL	0	NULL	HaeIII restriction fragments 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The base compositions proximal to the 5 ' ends of mRNA 's from promoters on these DNA fragments were elucidated by the polymerase initiation assay , in which the addition of various combinations of nucleoside triphosphates to the reaction allowed RNA polymerase to form high-salt-resistant initiation complexes with some of the known SmaI + EcoRI , EcoRI + HindIII , or HaeIII restriction fragments of lambda rifd 18 DNA .
	manualset3
142813	15	408942	5	NULL	NULL	0	NULL	lambda rifd 18 DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The base compositions proximal to the 5 ' ends of mRNA 's from promoters on these DNA fragments were elucidated by the polymerase initiation assay , in which the addition of various combinations of nucleoside triphosphates to the reaction allowed RNA polymerase to form high-salt-resistant initiation complexes with some of the known SmaI + EcoRI , EcoRI + HindIII , or HaeIII restriction fragments of lambda rifd 18 DNA .
	manualset3
142814	1	408943	5	NULL	NULL	0	NULL	base	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The base of bicuculline was less potent in blocking the slow afterhyperpolarization .
	manualset3
142815	2	408943	5	NULL	NULL	0	NULL	bicuculline 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The base of bicuculline was less potent in blocking the slow afterhyperpolarization .
	manualset3
142816	3	408943	5	NULL	NULL	NULL	NULL	afterhyperpolarization	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The base of bicuculline was less potent in blocking the slow afterhyperpolarization .
	manualset3
142817	1	408944	5	NULL	NULL	0	NULL	baseline rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The baseline rate of GIB in all studied populations rises markedly with advancing age .
	manualset3
142818	2	408944	5	NULL	NULL	0	NULL	GIB 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The baseline rate of GIB in all studied populations rises markedly with advancing age .
	manualset3
142819	3	408944	5	NULL	NULL	0	NULL	populations 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The baseline rate of GIB in all studied populations rises markedly with advancing age .
	manualset3
147967	4	408944	5	NULL	NULL	0	NULL	age 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The baseline rate of GIB in all studied populations rises markedly with advancing age .
	manualset3
142820	1	408945	5	NULL	NULL	0	NULL	basic mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The basic mechanism is destruction of neurons of the enteric nervous system .
	manualset3
142821	2	408945	5	NULL	NULL	0	NULL	destruction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The basic mechanism is destruction of neurons of the enteric nervous system .
	manualset3
142822	3	408945	5	NULL	NULL	0	NULL	neurons 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The basic mechanism is destruction of neurons of the enteric nervous system .
	manualset3
142823	4	408945	5	NULL	NULL	0	NULL	enteric nervous system 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The basic mechanism is destruction of neurons of the enteric nervous system .
	manualset3
142824	1	408946	5	NULL	NULL	0	NULL	basic parameters	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The basic parameters of growth and normal or altered gravitropical behavior of hairy roots are for the first time presented in this paper together with an ultrastructural and morphological analysis of the root statocytes .
	manualset3
142825	2	408946	5	NULL	NULL	0	NULL	growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The basic parameters of growth and normal or altered gravitropical behavior of hairy roots are for the first time presented in this paper together with an ultrastructural and morphological analysis of the root statocytes .
	manualset3
142826	3	408946	5	NULL	NULL	0	NULL	normal or altered gravitropical behavior	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The basic parameters of growth and normal or altered gravitropical behavior of hairy roots are for the first time presented in this paper together with an ultrastructural and morphological analysis of the root statocytes .
	manualset3
142827	4	408946	5	NULL	NULL	0	NULL	hairy roots	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The basic parameters of growth and normal or altered gravitropical behavior of hairy roots are for the first time presented in this paper together with an ultrastructural and morphological analysis of the root statocytes .
	manualset3
142828	5	408946	5	NULL	NULL	0	NULL	first time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The basic parameters of growth and normal or altered gravitropical behavior of hairy roots are for the first time presented in this paper together with an ultrastructural and morphological analysis of the root statocytes .
	manualset3
142829	6	408946	5	NULL	NULL	0	NULL	paper 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The basic parameters of growth and normal or altered gravitropical behavior of hairy roots are for the first time presented in this paper together with an ultrastructural and morphological analysis of the root statocytes .
	manualset3
142830	7	408946	5	NULL	NULL	0	NULL	ultrastructural analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The basic parameters of growth and normal or altered gravitropical behavior of hairy roots are for the first time presented in this paper together with an ultrastructural and morphological analysis of the root statocytes .
	manualset3
142831	8	408946	5	NULL	NULL	0	NULL	morphological analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The basic parameters of growth and normal or altered gravitropical behavior of hairy roots are for the first time presented in this paper together with an ultrastructural and morphological analysis of the root statocytes .
	manualset3
147968	9	408946	5	NULL	NULL	0	NULL	root statocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The basic parameters of growth and normal or altered gravitropical behavior of hairy roots are for the first time presented in this paper together with an ultrastructural and morphological analysis of the root statocytes .
	manualset3
142832	1	408947	5	NULL	NULL	0	NULL	basic patterns	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The basic patterns of student activities in the library , resources used to find current information , and resources anticipated for future education needs remained unchanged .
	manualset3
142833	2	408947	5	NULL	NULL	0	NULL	student activities 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The basic patterns of student activities in the library , resources used to find current information , and resources anticipated for future education needs remained unchanged .
	manualset3
142834	3	408947	5	NULL	NULL	0	NULL	library 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The basic patterns of student activities in the library , resources used to find current information , and resources anticipated for future education needs remained unchanged .
	manualset3
142835	4	408947	5	NULL	NULL	0	NULL	resources 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The basic patterns of student activities in the library , resources used to find current information , and resources anticipated for future education needs remained unchanged .
	manualset3
142836	5	408947	5	NULL	NULL	0	NULL	current information 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The basic patterns of student activities in the library , resources used to find current information , and resources anticipated for future education needs remained unchanged .
	manualset3
142837	6	408947	5	NULL	NULL	0	NULL	resources 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The basic patterns of student activities in the library , resources used to find current information , and resources anticipated for future education needs remained unchanged .
	manualset3
142838	7	408947	5	NULL	NULL	0	NULL	future education	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The basic patterns of student activities in the library , resources used to find current information , and resources anticipated for future education needs remained unchanged .
	manualset3
142839	1	408948	5	NULL	NULL	NULL	NULL	basic scales of interest 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The basic scales of interest lie in the lower-frequency domain , involving periods of fluctuations longer than tens of minutes .
	manualset3
142840	2	408948	5	NULL	NULL	0	NULL	lower-frequency domain	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The basic scales of interest lie in the lower-frequency domain , involving periods of fluctuations longer than tens of minutes .
	manualset3
142841	3	408948	5	NULL	NULL	0	NULL	periods 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The basic scales of interest lie in the lower-frequency domain , involving periods of fluctuations longer than tens of minutes .
	manualset3
142842	4	408948	5	NULL	NULL	0	NULL	fluctuations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The basic scales of interest lie in the lower-frequency domain , involving periods of fluctuations longer than tens of minutes .
	manualset3
142843	5	408948	5	NULL	NULL	0	NULL	tens of minutes	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The basic scales of interest lie in the lower-frequency domain , involving periods of fluctuations longer than tens of minutes .
	manualset3
142844	1	408949	5	NULL	NULL	0	NULL	basic thesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The basic thesis is that consciousness involves brain activities coupled to self-organizing ripples in fundamental reality .
	manualset3
142845	2	408949	5	NULL	NULL	0	NULL	consciousness 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The basic thesis is that consciousness involves brain activities coupled to self-organizing ripples in fundamental reality .
	manualset3
142846	3	408949	5	NULL	NULL	0	NULL	brain activities 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The basic thesis is that consciousness involves brain activities coupled to self-organizing ripples in fundamental reality .
	manualset3
142847	4	408949	5	NULL	NULL	0	NULL	self-organizing ripples	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The basic thesis is that consciousness involves brain activities coupled to self-organizing ripples in fundamental reality .
	manualset3
142848	5	408949	5	NULL	NULL	0	NULL	fundamental reality	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The basic thesis is that consciousness involves brain activities coupled to self-organizing ripples in fundamental reality .
	manualset3
142849	1	408950	5	NULL	NULL	0	NULL	enzyme immunoassay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A sensitive and specific enzyme immunoassay for bovine osteocalcin was developed with the use of enzyme-labeled antigen .
	manualset3
142850	2	408950	5	NULL	NULL	0	NULL	bovine osteocalcin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A sensitive and specific enzyme immunoassay for bovine osteocalcin was developed with the use of enzyme-labeled antigen .
	manualset3
142851	3	408950	5	NULL	NULL	0	NULL	use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A sensitive and specific enzyme immunoassay for bovine osteocalcin was developed with the use of enzyme-labeled antigen .
	manualset3
142852	4	408950	5	NULL	NULL	0	NULL	enzyme-labeled antigen	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A sensitive and specific enzyme immunoassay for bovine osteocalcin was developed with the use of enzyme-labeled antigen .
	manualset3
142853	1	408951	5	NULL	NULL	0	NULL	basis 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The basis for interindividual differences in asparaginase sensitivity remains unclear .
	manualset3
142854	2	408951	5	NULL	NULL	0	NULL	interindividual differences	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The basis for interindividual differences in asparaginase sensitivity remains unclear .
	manualset3
142855	3	408951	5	NULL	NULL	0	NULL	asparaginase sensitivity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The basis for interindividual differences in asparaginase sensitivity remains unclear .
	manualset3
142856	1	408952	5	NULL	NULL	0	NULL	basis 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The basis set effect on both the polarizabilities and hyperpolarizabilities of the studied systems has been explicitly taken into account relying on the augmented correlation consistent aug-cc-pVnZ ( n = D , T , Q , and 5 ) basis sets series .
	manualset3
142857	2	408952	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The basis set effect on both the polarizabilities and hyperpolarizabilities of the studied systems has been explicitly taken into account relying on the augmented correlation consistent aug-cc-pVnZ ( n = D , T , Q , and 5 ) basis sets series .
	manualset3
142858	3	408952	5	NULL	NULL	0	NULL	polarizabilities 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The basis set effect on both the polarizabilities and hyperpolarizabilities of the studied systems has been explicitly taken into account relying on the augmented correlation consistent aug-cc-pVnZ ( n = D , T , Q , and 5 ) basis sets series .
	manualset3
142859	4	408952	5	NULL	NULL	0	NULL	hyperpolarizabilities 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The basis set effect on both the polarizabilities and hyperpolarizabilities of the studied systems has been explicitly taken into account relying on the augmented correlation consistent aug-cc-pVnZ ( n = D , T , Q , and 5 ) basis sets series .
	manualset3
142860	5	408952	5	NULL	NULL	0	NULL	studied systems	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The basis set effect on both the polarizabilities and hyperpolarizabilities of the studied systems has been explicitly taken into account relying on the augmented correlation consistent aug-cc-pVnZ ( n = D , T , Q , and 5 ) basis sets series .
	manualset3
142861	6	408952	5	NULL	NULL	0	NULL	account 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The basis set effect on both the polarizabilities and hyperpolarizabilities of the studied systems has been explicitly taken into account relying on the augmented correlation consistent aug-cc-pVnZ ( n = D , T , Q , and 5 ) basis sets series .
	manualset3
142862	7	408952	5	NULL	NULL	0	NULL	augmented correlation consistent aug-cc-pVnZ ( n = D , T , Q , and 5 ) basis sets series	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The basis set effect on both the polarizabilities and hyperpolarizabilities of the studied systems has been explicitly taken into account relying on the augmented correlation consistent aug-cc-pVnZ ( n = D , T , Q , and 5 ) basis sets series .
	manualset3
142863	1	408953	5	NULL	NULL	0	NULL	basophil proteoglycans	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The basophil proteoglycans and glycosaminoglycans were capable of binding histamine in water , but not in phosphate-buffered saline , and had no anticoagulant activity .
	manualset3
142864	2	408953	5	NULL	NULL	0	NULL	glycosaminoglycans 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The basophil proteoglycans and glycosaminoglycans were capable of binding histamine in water , but not in phosphate-buffered saline , and had no anticoagulant activity .
	manualset3
142865	3	408953	5	NULL	NULL	0	NULL	histamine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The basophil proteoglycans and glycosaminoglycans were capable of binding histamine in water , but not in phosphate-buffered saline , and had no anticoagulant activity .
	manualset3
142866	4	408953	5	NULL	NULL	0	NULL	water 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The basophil proteoglycans and glycosaminoglycans were capable of binding histamine in water , but not in phosphate-buffered saline , and had no anticoagulant activity .
	manualset3
142867	5	408953	5	NULL	NULL	0	NULL	phosphate-buffered saline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The basophil proteoglycans and glycosaminoglycans were capable of binding histamine in water , but not in phosphate-buffered saline , and had no anticoagulant activity .
	manualset3
142868	6	408953	5	NULL	NULL	0	NULL	anticoagulant activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The basophil proteoglycans and glycosaminoglycans were capable of binding histamine in water , but not in phosphate-buffered saline , and had no anticoagulant activity .
	manualset3
142869	1	408954	5	NULL	NULL	0	NULL	bcl-2 Mbr	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The bcl-2 Mbr assumes a non-B DNA conformation , thus explaining its distinctive fragility .
	manualset3
142870	2	408954	5	NULL	NULL	0	NULL	non-B DNA conformation	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The bcl-2 Mbr assumes a non-B DNA conformation , thus explaining its distinctive fragility .
	manualset3
142871	3	408954	5	NULL	NULL	0	NULL	fragility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The bcl-2 Mbr assumes a non-B DNA conformation , thus explaining its distinctive fragility .
	manualset3
142872	1	408955	5	NULL	NULL	0	NULL	beads 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The beads were used to inoculate leeks grown under standard conditions for 6 wk , then development of root colonization by G. intraradices was recorded .
	manualset3
142873	2	408955	5	NULL	NULL	0	NULL	leeks 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The beads were used to inoculate leeks grown under standard conditions for 6 wk , then development of root colonization by G. intraradices was recorded .
	manualset3
142874	3	408955	5	NULL	NULL	0	NULL	standard conditions	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The beads were used to inoculate leeks grown under standard conditions for 6 wk , then development of root colonization by G. intraradices was recorded .
	manualset3
142875	4	408955	5	NULL	NULL	0	NULL	6 wk	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The beads were used to inoculate leeks grown under standard conditions for 6 wk , then development of root colonization by G. intraradices was recorded .
	manualset3
142876	5	408955	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The beads were used to inoculate leeks grown under standard conditions for 6 wk , then development of root colonization by G. intraradices was recorded .
	manualset3
142877	6	408955	5	NULL	NULL	0	NULL	root colonization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The beads were used to inoculate leeks grown under standard conditions for 6 wk , then development of root colonization by G. intraradices was recorded .
	manualset3
142878	7	408955	5	NULL	NULL	0	NULL	G. intraradices	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The beads were used to inoculate leeks grown under standard conditions for 6 wk , then development of root colonization by G. intraradices was recorded .
	manualset3
142879	1	408956	5	NULL	NULL	0	NULL	behavior 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The behavior of the nonresonantly enhanced BP is comparable to that of the resonantly enhanced ZnTPP samples .
	manualset3
142880	2	408956	5	NULL	NULL	0	NULL	nonresonantly enhanced BP	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The behavior of the nonresonantly enhanced BP is comparable to that of the resonantly enhanced ZnTPP samples .
	manualset3
142881	3	408956	5	NULL	NULL	0	NULL	resonantly enhanced ZnTPP samples	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The behavior of the nonresonantly enhanced BP is comparable to that of the resonantly enhanced ZnTPP samples .
	manualset3
142900	1	408957	5	NULL	NULL	0	NULL	behavioral disruption	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The behavioral disruption was suggested to result , at least in part , from a dopaminergic disturbance , since the behavior was restored by the administration of DOPA or apomorphine but not by 5-hydroxytryptophan .
	manualset3
142901	2	408957	5	NULL	NULL	0	NULL	dopaminergic disturbance	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The behavioral disruption was suggested to result , at least in part , from a dopaminergic disturbance , since the behavior was restored by the administration of DOPA or apomorphine but not by 5-hydroxytryptophan .
	manualset3
142902	3	408957	5	NULL	NULL	0	NULL	behavior 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The behavioral disruption was suggested to result , at least in part , from a dopaminergic disturbance , since the behavior was restored by the administration of DOPA or apomorphine but not by 5-hydroxytryptophan .
	manualset3
142903	4	408957	5	NULL	NULL	0	NULL	administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The behavioral disruption was suggested to result , at least in part , from a dopaminergic disturbance , since the behavior was restored by the administration of DOPA or apomorphine but not by 5-hydroxytryptophan .
	manualset3
142904	5	408957	5	NULL	NULL	0	NULL	DOPA 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The behavioral disruption was suggested to result , at least in part , from a dopaminergic disturbance , since the behavior was restored by the administration of DOPA or apomorphine but not by 5-hydroxytryptophan .
	manualset3
142905	6	408957	5	NULL	NULL	0	NULL	apomorphine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The behavioral disruption was suggested to result , at least in part , from a dopaminergic disturbance , since the behavior was restored by the administration of DOPA or apomorphine but not by 5-hydroxytryptophan .
	manualset3
142906	7	408957	5	NULL	NULL	0	NULL	5-hydroxytryptophan	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The behavioral disruption was suggested to result , at least in part , from a dopaminergic disturbance , since the behavior was restored by the administration of DOPA or apomorphine but not by 5-hydroxytryptophan .
	manualset3
142907	2	408958	5	NULL	NULL	NULL	NULL	central dimers	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The bend in the central dimers is distributed to some extent between the adjacent links , though the main fraction of the bend remains within the central link .
	manualset3
142908	3	408958	5	NULL	NULL	NULL	NULL	adjacent links	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The bend in the central dimers is distributed to some extent between the adjacent links , though the main fraction of the bend remains within the central link .
	manualset3
142909	4	408958	5	NULL	NULL	NULL	NULL	fraction 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The bend in the central dimers is distributed to some extent between the adjacent links , though the main fraction of the bend remains within the central link .
	manualset3
142910	5	408958	5	NULL	NULL	NULL	NULL	bend 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The bend in the central dimers is distributed to some extent between the adjacent links , though the main fraction of the bend remains within the central link .
	manualset3
142911	6	408958	5	NULL	NULL	0	NULL	central link	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The bend in the central dimers is distributed to some extent between the adjacent links , though the main fraction of the bend remains within the central link .
	manualset3
142912	1	408958	5	NULL	NULL	0	NULL	bend 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The bend in the central dimers is distributed to some extent between the adjacent links , though the main fraction of the bend remains within the central link .
	manualset3
142913	1	408959	5	NULL	NULL	NULL	NULL	beneficial effect	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The beneficial effect of mAb antimetastatic therapy was found to be useful against several syngeneic melanomas , including JB/MS , B16 and several sublines of the B16 F10 melanoma .
	manualset3
142914	2	408959	5	NULL	NULL	0	NULL	mAb antimetastatic therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial effect of mAb antimetastatic therapy was found to be useful against several syngeneic melanomas , including JB/MS , B16 and several sublines of the B16 F10 melanoma .
	manualset3
142915	3	408959	5	NULL	NULL	0	NULL	syngeneic melanomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial effect of mAb antimetastatic therapy was found to be useful against several syngeneic melanomas , including JB/MS , B16 and several sublines of the B16 F10 melanoma .
	manualset3
142916	4	408959	5	NULL	NULL	NULL	NULL	JB/MS melanoma	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The beneficial effect of mAb antimetastatic therapy was found to be useful against several syngeneic melanomas , including JB/MS , B16 and several sublines of the B16 F10 melanoma .
	manualset3
142917	5	408959	5	NULL	NULL	NULL	NULL	B16 melanoma	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The beneficial effect of mAb antimetastatic therapy was found to be useful against several syngeneic melanomas , including JB/MS , B16 and several sublines of the B16 F10 melanoma .
	manualset3
142918	6	408959	5	NULL	NULL	0	NULL	sublines of the B16 F10 melanoma	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial effect of mAb antimetastatic therapy was found to be useful against several syngeneic melanomas , including JB/MS , B16 and several sublines of the B16 F10 melanoma .
	manualset3
142919	1	408960	5	NULL	NULL	0	NULL	specific method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A sensitive and specific method for the simultaneous quantitation of ifosfamide ( IF ) , 4-hydroxylifosfamide ( 4-OHIF ) , N2-dechloroethylifosfamide ( N2D ) , N3-dechloroethylifosfamide ( N3D ) and iphosphoramide mustard ( IPM ) has been developed using gas chromatography-mass spectrometry ( GC-MS ) with an ion-trap mass spectrometer .
	manualset3
142920	2	408960	5	NULL	NULL	0	NULL	simultaneous quantitation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A sensitive and specific method for the simultaneous quantitation of ifosfamide ( IF ) , 4-hydroxylifosfamide ( 4-OHIF ) , N2-dechloroethylifosfamide ( N2D ) , N3-dechloroethylifosfamide ( N3D ) and iphosphoramide mustard ( IPM ) has been developed using gas chromatography-mass spectrometry ( GC-MS ) with an ion-trap mass spectrometer .
	manualset3
142921	3	408960	5	NULL	NULL	0	NULL	ifosfamide ( IF ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A sensitive and specific method for the simultaneous quantitation of ifosfamide ( IF ) , 4-hydroxylifosfamide ( 4-OHIF ) , N2-dechloroethylifosfamide ( N2D ) , N3-dechloroethylifosfamide ( N3D ) and iphosphoramide mustard ( IPM ) has been developed using gas chromatography-mass spectrometry ( GC-MS ) with an ion-trap mass spectrometer .
	manualset3
142922	4	408960	5	NULL	NULL	0	NULL	4-hydroxylifosfamide ( 4-OHIF )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A sensitive and specific method for the simultaneous quantitation of ifosfamide ( IF ) , 4-hydroxylifosfamide ( 4-OHIF ) , N2-dechloroethylifosfamide ( N2D ) , N3-dechloroethylifosfamide ( N3D ) and iphosphoramide mustard ( IPM ) has been developed using gas chromatography-mass spectrometry ( GC-MS ) with an ion-trap mass spectrometer .
	manualset3
142923	5	408960	5	NULL	NULL	0	NULL	 N2-dechloroethylifosfamide ( N2D )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A sensitive and specific method for the simultaneous quantitation of ifosfamide ( IF ) , 4-hydroxylifosfamide ( 4-OHIF ) , N2-dechloroethylifosfamide ( N2D ) , N3-dechloroethylifosfamide ( N3D ) and iphosphoramide mustard ( IPM ) has been developed using gas chromatography-mass spectrometry ( GC-MS ) with an ion-trap mass spectrometer .
	manualset3
142924	6	408960	5	NULL	NULL	0	NULL	N3-dechloroethylifosfamide ( N3D )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A sensitive and specific method for the simultaneous quantitation of ifosfamide ( IF ) , 4-hydroxylifosfamide ( 4-OHIF ) , N2-dechloroethylifosfamide ( N2D ) , N3-dechloroethylifosfamide ( N3D ) and iphosphoramide mustard ( IPM ) has been developed using gas chromatography-mass spectrometry ( GC-MS ) with an ion-trap mass spectrometer .
	manualset3
142925	7	408960	5	NULL	NULL	0	NULL	iphosphoramide mustard ( IPM ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A sensitive and specific method for the simultaneous quantitation of ifosfamide ( IF ) , 4-hydroxylifosfamide ( 4-OHIF ) , N2-dechloroethylifosfamide ( N2D ) , N3-dechloroethylifosfamide ( N3D ) and iphosphoramide mustard ( IPM ) has been developed using gas chromatography-mass spectrometry ( GC-MS ) with an ion-trap mass spectrometer .
	manualset3
142926	8	408960	5	NULL	NULL	0	NULL	 gas chromatography-mass spectrometry ( GC-MS )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A sensitive and specific method for the simultaneous quantitation of ifosfamide ( IF ) , 4-hydroxylifosfamide ( 4-OHIF ) , N2-dechloroethylifosfamide ( N2D ) , N3-dechloroethylifosfamide ( N3D ) and iphosphoramide mustard ( IPM ) has been developed using gas chromatography-mass spectrometry ( GC-MS ) with an ion-trap mass spectrometer .
	manualset3
142927	9	408960	5	NULL	NULL	0	NULL	ion-trap mass spectrometer	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A sensitive and specific method for the simultaneous quantitation of ifosfamide ( IF ) , 4-hydroxylifosfamide ( 4-OHIF ) , N2-dechloroethylifosfamide ( N2D ) , N3-dechloroethylifosfamide ( N3D ) and iphosphoramide mustard ( IPM ) has been developed using gas chromatography-mass spectrometry ( GC-MS ) with an ion-trap mass spectrometer .
	manualset3
142928	1	408961	5	NULL	NULL	0	NULL	beneficial effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial effects of CT-containing forages on the ability of young deer to manage internal parasite infections could be due to : indirect effects of CT resulting in increased amino-acid absorption , better meeting demands of the immune system ; direct inhibitory effects of CT on parasite larvae and ; taller plant morphology , reducing the ingestion of infective larvae .
	manualset3
142929	2	408961	5	NULL	NULL	0	NULL	CT-containing forages	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial effects of CT-containing forages on the ability of young deer to manage internal parasite infections could be due to : indirect effects of CT resulting in increased amino-acid absorption , better meeting demands of the immune system ; direct inhibitory effects of CT on parasite larvae and ; taller plant morphology , reducing the ingestion of infective larvae .
	manualset3
142930	3	408961	5	NULL	NULL	0	NULL	ability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial effects of CT-containing forages on the ability of young deer to manage internal parasite infections could be due to : indirect effects of CT resulting in increased amino-acid absorption , better meeting demands of the immune system ; direct inhibitory effects of CT on parasite larvae and ; taller plant morphology , reducing the ingestion of infective larvae .
	manualset3
142931	4	408961	5	NULL	NULL	0	NULL	young deer	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial effects of CT-containing forages on the ability of young deer to manage internal parasite infections could be due to : indirect effects of CT resulting in increased amino-acid absorption , better meeting demands of the immune system ; direct inhibitory effects of CT on parasite larvae and ; taller plant morphology , reducing the ingestion of infective larvae .
	manualset3
142932	5	408961	5	NULL	NULL	0	NULL	internal parasite infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial effects of CT-containing forages on the ability of young deer to manage internal parasite infections could be due to : indirect effects of CT resulting in increased amino-acid absorption , better meeting demands of the immune system ; direct inhibitory effects of CT on parasite larvae and ; taller plant morphology , reducing the ingestion of infective larvae .
	manualset3
142933	6	408961	5	NULL	NULL	0	NULL	indirect effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial effects of CT-containing forages on the ability of young deer to manage internal parasite infections could be due to : indirect effects of CT resulting in increased amino-acid absorption , better meeting demands of the immune system ; direct inhibitory effects of CT on parasite larvae and ; taller plant morphology , reducing the ingestion of infective larvae .
	manualset3
142934	7	408961	5	NULL	NULL	0	NULL	CT 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial effects of CT-containing forages on the ability of young deer to manage internal parasite infections could be due to : indirect effects of CT resulting in increased amino-acid absorption , better meeting demands of the immune system ; direct inhibitory effects of CT on parasite larvae and ; taller plant morphology , reducing the ingestion of infective larvae .
	manualset3
142935	8	408961	5	NULL	NULL	0	NULL	amino-acid absorption	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial effects of CT-containing forages on the ability of young deer to manage internal parasite infections could be due to : indirect effects of CT resulting in increased amino-acid absorption , better meeting demands of the immune system ; direct inhibitory effects of CT on parasite larvae and ; taller plant morphology , reducing the ingestion of infective larvae .
	manualset3
142936	9	408961	5	NULL	NULL	NULL	NULL	demands	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The beneficial effects of CT-containing forages on the ability of young deer to manage internal parasite infections could be due to : indirect effects of CT resulting in increased amino-acid absorption , better meeting demands of the immune system ; direct inhibitory effects of CT on parasite larvae and ; taller plant morphology , reducing the ingestion of infective larvae .
	manualset3
142937	10	408961	5	NULL	NULL	0	NULL	immune system	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial effects of CT-containing forages on the ability of young deer to manage internal parasite infections could be due to : indirect effects of CT resulting in increased amino-acid absorption , better meeting demands of the immune system ; direct inhibitory effects of CT on parasite larvae and ; taller plant morphology , reducing the ingestion of infective larvae .
	manualset3
142938	11	408961	5	NULL	NULL	0	NULL	direct inhibitory effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial effects of CT-containing forages on the ability of young deer to manage internal parasite infections could be due to : indirect effects of CT resulting in increased amino-acid absorption , better meeting demands of the immune system ; direct inhibitory effects of CT on parasite larvae and ; taller plant morphology , reducing the ingestion of infective larvae .
	manualset3
142939	12	408961	5	NULL	NULL	0	NULL	CT 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial effects of CT-containing forages on the ability of young deer to manage internal parasite infections could be due to : indirect effects of CT resulting in increased amino-acid absorption , better meeting demands of the immune system ; direct inhibitory effects of CT on parasite larvae and ; taller plant morphology , reducing the ingestion of infective larvae .
	manualset3
142940	13	408961	5	NULL	NULL	0	NULL	parasite larvae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial effects of CT-containing forages on the ability of young deer to manage internal parasite infections could be due to : indirect effects of CT resulting in increased amino-acid absorption , better meeting demands of the immune system ; direct inhibitory effects of CT on parasite larvae and ; taller plant morphology , reducing the ingestion of infective larvae .
	manualset3
142941	14	408961	5	NULL	NULL	0	NULL	taller plant morphology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial effects of CT-containing forages on the ability of young deer to manage internal parasite infections could be due to : indirect effects of CT resulting in increased amino-acid absorption , better meeting demands of the immune system ; direct inhibitory effects of CT on parasite larvae and ; taller plant morphology , reducing the ingestion of infective larvae .
	manualset3
142942	15	408961	5	NULL	NULL	0	NULL	ingestion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial effects of CT-containing forages on the ability of young deer to manage internal parasite infections could be due to : indirect effects of CT resulting in increased amino-acid absorption , better meeting demands of the immune system ; direct inhibitory effects of CT on parasite larvae and ; taller plant morphology , reducing the ingestion of infective larvae .
	manualset3
142943	16	408961	5	NULL	NULL	0	NULL	infective larvae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial effects of CT-containing forages on the ability of young deer to manage internal parasite infections could be due to : indirect effects of CT resulting in increased amino-acid absorption , better meeting demands of the immune system ; direct inhibitory effects of CT on parasite larvae and ; taller plant morphology , reducing the ingestion of infective larvae .
	manualset3
142944	1	408962	5	NULL	NULL	NULL	NULL	beneficial interactions	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The beneficial interactions between antiarrhythmic drugs and an ICD are slowing of ventricular tachycardia , which yields improved hemodynamic tolerance ; improved antitachycardia pacing and low energy cardioversion success ; lowering of antiarrhythmic drug doses , which reduces the risk of side effects ; limiting the number of arrhythmia episodes , which minimizes patients discomfort and prolongs ICD battery life ; and preventing or slowing supraventricular tachyarrhythmias , which reduces the number of inappropriate shocks from the ICD .
	manualset3
142945	2	408962	5	NULL	NULL	0	NULL	antiarrhythmic drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial interactions between antiarrhythmic drugs and an ICD are slowing of ventricular tachycardia , which yields improved hemodynamic tolerance ; improved antitachycardia pacing and low energy cardioversion success ; lowering of antiarrhythmic drug doses , which reduces the risk of side effects ; limiting the number of arrhythmia episodes , which minimizes patients discomfort and prolongs ICD battery life ; and preventing or slowing supraventricular tachyarrhythmias , which reduces the number of inappropriate shocks from the ICD .
	manualset3
142946	3	408962	5	NULL	NULL	0	NULL	ICD 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial interactions between antiarrhythmic drugs and an ICD are slowing of ventricular tachycardia , which yields improved hemodynamic tolerance ; improved antitachycardia pacing and low energy cardioversion success ; lowering of antiarrhythmic drug doses , which reduces the risk of side effects ; limiting the number of arrhythmia episodes , which minimizes patients discomfort and prolongs ICD battery life ; and preventing or slowing supraventricular tachyarrhythmias , which reduces the number of inappropriate shocks from the ICD .
	manualset3
142947	4	408962	5	NULL	NULL	0	NULL	ventricular tachycardia	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial interactions between antiarrhythmic drugs and an ICD are slowing of ventricular tachycardia , which yields improved hemodynamic tolerance ; improved antitachycardia pacing and low energy cardioversion success ; lowering of antiarrhythmic drug doses , which reduces the risk of side effects ; limiting the number of arrhythmia episodes , which minimizes patients discomfort and prolongs ICD battery life ; and preventing or slowing supraventricular tachyarrhythmias , which reduces the number of inappropriate shocks from the ICD .
	manualset3
142948	5	408962	5	NULL	NULL	0	NULL	improved hemodynamic tolerance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial interactions between antiarrhythmic drugs and an ICD are slowing of ventricular tachycardia , which yields improved hemodynamic tolerance ; improved antitachycardia pacing and low energy cardioversion success ; lowering of antiarrhythmic drug doses , which reduces the risk of side effects ; limiting the number of arrhythmia episodes , which minimizes patients discomfort and prolongs ICD battery life ; and preventing or slowing supraventricular tachyarrhythmias , which reduces the number of inappropriate shocks from the ICD .
	manualset3
142949	6	408962	5	NULL	NULL	0	NULL	improved antitachycardia pacing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial interactions between antiarrhythmic drugs and an ICD are slowing of ventricular tachycardia , which yields improved hemodynamic tolerance ; improved antitachycardia pacing and low energy cardioversion success ; lowering of antiarrhythmic drug doses , which reduces the risk of side effects ; limiting the number of arrhythmia episodes , which minimizes patients discomfort and prolongs ICD battery life ; and preventing or slowing supraventricular tachyarrhythmias , which reduces the number of inappropriate shocks from the ICD .
	manualset3
142950	7	408962	5	NULL	NULL	0	NULL	low energy cardioversion success	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial interactions between antiarrhythmic drugs and an ICD are slowing of ventricular tachycardia , which yields improved hemodynamic tolerance ; improved antitachycardia pacing and low energy cardioversion success ; lowering of antiarrhythmic drug doses , which reduces the risk of side effects ; limiting the number of arrhythmia episodes , which minimizes patients discomfort and prolongs ICD battery life ; and preventing or slowing supraventricular tachyarrhythmias , which reduces the number of inappropriate shocks from the ICD .
	manualset3
142951	8	408962	5	NULL	NULL	0	NULL	antiarrhythmic drug doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial interactions between antiarrhythmic drugs and an ICD are slowing of ventricular tachycardia , which yields improved hemodynamic tolerance ; improved antitachycardia pacing and low energy cardioversion success ; lowering of antiarrhythmic drug doses , which reduces the risk of side effects ; limiting the number of arrhythmia episodes , which minimizes patients discomfort and prolongs ICD battery life ; and preventing or slowing supraventricular tachyarrhythmias , which reduces the number of inappropriate shocks from the ICD .
	manualset3
142952	9	408962	5	NULL	NULL	0	NULL	risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial interactions between antiarrhythmic drugs and an ICD are slowing of ventricular tachycardia , which yields improved hemodynamic tolerance ; improved antitachycardia pacing and low energy cardioversion success ; lowering of antiarrhythmic drug doses , which reduces the risk of side effects ; limiting the number of arrhythmia episodes , which minimizes patients discomfort and prolongs ICD battery life ; and preventing or slowing supraventricular tachyarrhythmias , which reduces the number of inappropriate shocks from the ICD .
	manualset3
142953	10	408962	5	NULL	NULL	0	NULL	side effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial interactions between antiarrhythmic drugs and an ICD are slowing of ventricular tachycardia , which yields improved hemodynamic tolerance ; improved antitachycardia pacing and low energy cardioversion success ; lowering of antiarrhythmic drug doses , which reduces the risk of side effects ; limiting the number of arrhythmia episodes , which minimizes patients discomfort and prolongs ICD battery life ; and preventing or slowing supraventricular tachyarrhythmias , which reduces the number of inappropriate shocks from the ICD .
	manualset3
142954	11	408962	5	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial interactions between antiarrhythmic drugs and an ICD are slowing of ventricular tachycardia , which yields improved hemodynamic tolerance ; improved antitachycardia pacing and low energy cardioversion success ; lowering of antiarrhythmic drug doses , which reduces the risk of side effects ; limiting the number of arrhythmia episodes , which minimizes patients discomfort and prolongs ICD battery life ; and preventing or slowing supraventricular tachyarrhythmias , which reduces the number of inappropriate shocks from the ICD .
	manualset3
142955	12	408962	5	NULL	NULL	NULL	NULL	arrhythmia episodes	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The beneficial interactions between antiarrhythmic drugs and an ICD are slowing of ventricular tachycardia , which yields improved hemodynamic tolerance ; improved antitachycardia pacing and low energy cardioversion success ; lowering of antiarrhythmic drug doses , which reduces the risk of side effects ; limiting the number of arrhythmia episodes , which minimizes patients discomfort and prolongs ICD battery life ; and preventing or slowing supraventricular tachyarrhythmias , which reduces the number of inappropriate shocks from the ICD .
	manualset3
142956	13	408962	5	NULL	NULL	0	NULL	patients discomfort	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial interactions between antiarrhythmic drugs and an ICD are slowing of ventricular tachycardia , which yields improved hemodynamic tolerance ; improved antitachycardia pacing and low energy cardioversion success ; lowering of antiarrhythmic drug doses , which reduces the risk of side effects ; limiting the number of arrhythmia episodes , which minimizes patients discomfort and prolongs ICD battery life ; and preventing or slowing supraventricular tachyarrhythmias , which reduces the number of inappropriate shocks from the ICD .
	manualset3
142957	14	408962	5	NULL	NULL	0	NULL	ICD battery life 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial interactions between antiarrhythmic drugs and an ICD are slowing of ventricular tachycardia , which yields improved hemodynamic tolerance ; improved antitachycardia pacing and low energy cardioversion success ; lowering of antiarrhythmic drug doses , which reduces the risk of side effects ; limiting the number of arrhythmia episodes , which minimizes patients discomfort and prolongs ICD battery life ; and preventing or slowing supraventricular tachyarrhythmias , which reduces the number of inappropriate shocks from the ICD .
	manualset3
142958	15	408962	5	NULL	NULL	0	NULL	supraventricular tachyarrhythmias	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial interactions between antiarrhythmic drugs and an ICD are slowing of ventricular tachycardia , which yields improved hemodynamic tolerance ; improved antitachycardia pacing and low energy cardioversion success ; lowering of antiarrhythmic drug doses , which reduces the risk of side effects ; limiting the number of arrhythmia episodes , which minimizes patients discomfort and prolongs ICD battery life ; and preventing or slowing supraventricular tachyarrhythmias , which reduces the number of inappropriate shocks from the ICD .
	manualset3
142959	16	408962	5	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial interactions between antiarrhythmic drugs and an ICD are slowing of ventricular tachycardia , which yields improved hemodynamic tolerance ; improved antitachycardia pacing and low energy cardioversion success ; lowering of antiarrhythmic drug doses , which reduces the risk of side effects ; limiting the number of arrhythmia episodes , which minimizes patients discomfort and prolongs ICD battery life ; and preventing or slowing supraventricular tachyarrhythmias , which reduces the number of inappropriate shocks from the ICD .
	manualset3
142960	17	408962	5	NULL	NULL	0	NULL	inappropriate shocks 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial interactions between antiarrhythmic drugs and an ICD are slowing of ventricular tachycardia , which yields improved hemodynamic tolerance ; improved antitachycardia pacing and low energy cardioversion success ; lowering of antiarrhythmic drug doses , which reduces the risk of side effects ; limiting the number of arrhythmia episodes , which minimizes patients discomfort and prolongs ICD battery life ; and preventing or slowing supraventricular tachyarrhythmias , which reduces the number of inappropriate shocks from the ICD .
	manualset3
142961	18	408962	5	NULL	NULL	0	NULL	ICD 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The beneficial interactions between antiarrhythmic drugs and an ICD are slowing of ventricular tachycardia , which yields improved hemodynamic tolerance ; improved antitachycardia pacing and low energy cardioversion success ; lowering of antiarrhythmic drug doses , which reduces the risk of side effects ; limiting the number of arrhythmia episodes , which minimizes patients discomfort and prolongs ICD battery life ; and preventing or slowing supraventricular tachyarrhythmias , which reduces the number of inappropriate shocks from the ICD .
	manualset3
142962	1	408963	5	NULL	NULL	0	NULL	benefit 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The benefit of being a social butterfly : communal roosting deters predation .
	manualset3
142963	2	408963	5	NULL	NULL	0	NULL	social butterfly 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The benefit of being a social butterfly : communal roosting deters predation .
	manualset3
142964	3	408963	5	NULL	NULL	0	NULL	predation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The benefit of being a social butterfly : communal roosting deters predation .
	manualset3
142965	1	408964	5	NULL	NULL	0	NULL	analgesic effect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The best analgesic effect was in patients treated with intra-articular ketorolac , and this was statistically significant in : postoperative analgesic effect and the need for additional pain medication immediately after surgery , and after 24 h. No complications were found related to the intra-articular treatment .
	manualset3
142966	2	408964	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The best analgesic effect was in patients treated with intra-articular ketorolac , and this was statistically significant in : postoperative analgesic effect and the need for additional pain medication immediately after surgery , and after 24 h. No complications were found related to the intra-articular treatment .
	manualset3
142967	3	408964	5	NULL	NULL	0	NULL	intra-articular ketorolac	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The best analgesic effect was in patients treated with intra-articular ketorolac , and this was statistically significant in : postoperative analgesic effect and the need for additional pain medication immediately after surgery , and after 24 h. No complications were found related to the intra-articular treatment .
	manualset3
142968	4	408964	5	NULL	NULL	0	NULL	postoperative analgesic effect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The best analgesic effect was in patients treated with intra-articular ketorolac , and this was statistically significant in : postoperative analgesic effect and the need for additional pain medication immediately after surgery , and after 24 h. No complications were found related to the intra-articular treatment .
	manualset3
142969	5	408964	5	NULL	NULL	NULL	NULL	additional pain medication	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The best analgesic effect was in patients treated with intra-articular ketorolac , and this was statistically significant in : postoperative analgesic effect and the need for additional pain medication immediately after surgery , and after 24 h. No complications were found related to the intra-articular treatment .
	manualset3
142970	6	408964	5	NULL	NULL	0	NULL	surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The best analgesic effect was in patients treated with intra-articular ketorolac , and this was statistically significant in : postoperative analgesic effect and the need for additional pain medication immediately after surgery , and after 24 h. No complications were found related to the intra-articular treatment .
	manualset3
142971	7	408964	5	NULL	NULL	0	NULL	24 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The best analgesic effect was in patients treated with intra-articular ketorolac , and this was statistically significant in : postoperative analgesic effect and the need for additional pain medication immediately after surgery , and after 24 h. No complications were found related to the intra-articular treatment .
	manualset3
142972	8	408964	5	NULL	NULL	0	NULL	complications 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The best analgesic effect was in patients treated with intra-articular ketorolac , and this was statistically significant in : postoperative analgesic effect and the need for additional pain medication immediately after surgery , and after 24 h. No complications were found related to the intra-articular treatment .
	manualset3
142973	9	408964	5	NULL	NULL	0	NULL	intra-articular treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The best analgesic effect was in patients treated with intra-articular ketorolac , and this was statistically significant in : postoperative analgesic effect and the need for additional pain medication immediately after surgery , and after 24 h. No complications were found related to the intra-articular treatment .
	manualset3
142974	1	408965	5	NULL	NULL	0	NULL	matching stimulation parameters 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The best matching stimulation parameters , from k = 68 different forms , are selected by the reinforcement learning algorithm consistently after 334 realizations .
	manualset3
142975	2	408965	5	NULL	NULL	0	NULL	k = 68 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The best matching stimulation parameters , from k = 68 different forms , are selected by the reinforcement learning algorithm consistently after 334 realizations .
	manualset3
142976	3	408965	5	NULL	NULL	0	NULL	reinforcement learning algorithm	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The best matching stimulation parameters , from k = 68 different forms , are selected by the reinforcement learning algorithm consistently after 334 realizations .
	manualset3
142977	4	408965	5	NULL	NULL	0	NULL	334 realizations	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The best matching stimulation parameters , from k = 68 different forms , are selected by the reinforcement learning algorithm consistently after 334 realizations .
	manualset3
142978	1	408966	5	NULL	NULL	0	NULL	( semipartial ) correlation coefficients	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The best part ( semipartial ) correlation coefficients predicting increasing CVP were identified with v-wave velocity ( 0.823 ) , S-wave velocity ( -0.800 ) , CVC diameter ( 0.855 ) , and hepatic vein diameter ( 0.815 ) .
	manualset3
142979	2	408966	5	NULL	NULL	0	NULL	CVP 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The best part ( semipartial ) correlation coefficients predicting increasing CVP were identified with v-wave velocity ( 0.823 ) , S-wave velocity ( -0.800 ) , CVC diameter ( 0.855 ) , and hepatic vein diameter ( 0.815 ) .
	manualset3
142980	3	408966	5	NULL	NULL	0	NULL	 v-wave velocity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The best part ( semipartial ) correlation coefficients predicting increasing CVP were identified with v-wave velocity ( 0.823 ) , S-wave velocity ( -0.800 ) , CVC diameter ( 0.855 ) , and hepatic vein diameter ( 0.815 ) .
	manualset3
142981	4	408966	5	NULL	NULL	0	NULL	 0.823 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The best part ( semipartial ) correlation coefficients predicting increasing CVP were identified with v-wave velocity ( 0.823 ) , S-wave velocity ( -0.800 ) , CVC diameter ( 0.855 ) , and hepatic vein diameter ( 0.815 ) .
	manualset3
142982	5	408966	5	NULL	NULL	0	NULL	S-wave velocity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The best part ( semipartial ) correlation coefficients predicting increasing CVP were identified with v-wave velocity ( 0.823 ) , S-wave velocity ( -0.800 ) , CVC diameter ( 0.855 ) , and hepatic vein diameter ( 0.815 ) .
	manualset3
142983	6	408966	5	NULL	NULL	0	NULL	 -0.800	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The best part ( semipartial ) correlation coefficients predicting increasing CVP were identified with v-wave velocity ( 0.823 ) , S-wave velocity ( -0.800 ) , CVC diameter ( 0.855 ) , and hepatic vein diameter ( 0.815 ) .
	manualset3
142984	7	408966	5	NULL	NULL	0	NULL	CVC diameter	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The best part ( semipartial ) correlation coefficients predicting increasing CVP were identified with v-wave velocity ( 0.823 ) , S-wave velocity ( -0.800 ) , CVC diameter ( 0.855 ) , and hepatic vein diameter ( 0.815 ) .
	manualset3
142985	8	408966	5	NULL	NULL	0	NULL	0.855	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The best part ( semipartial ) correlation coefficients predicting increasing CVP were identified with v-wave velocity ( 0.823 ) , S-wave velocity ( -0.800 ) , CVC diameter ( 0.855 ) , and hepatic vein diameter ( 0.815 ) .
	manualset3
142986	9	408966	5	NULL	NULL	0	NULL	hepatic vein diameter	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The best part ( semipartial ) correlation coefficients predicting increasing CVP were identified with v-wave velocity ( 0.823 ) , S-wave velocity ( -0.800 ) , CVC diameter ( 0.855 ) , and hepatic vein diameter ( 0.815 ) .
	manualset3
142987	10	408966	5	NULL	NULL	0	NULL	0.815	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The best part ( semipartial ) correlation coefficients predicting increasing CVP were identified with v-wave velocity ( 0.823 ) , S-wave velocity ( -0.800 ) , CVC diameter ( 0.855 ) , and hepatic vein diameter ( 0.815 ) .
	manualset3
142988	1	408967	5	NULL	NULL	0	NULL	members of the Cys-loop family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The best studied members of the Cys-loop family are nACh , 5-HT3 , GABAA and glycine receptors .
	manualset3
142989	2	408967	5	NULL	NULL	0	NULL	nACh receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The best studied members of the Cys-loop family are nACh , 5-HT3 , GABAA and glycine receptors .
	manualset3
142990	3	408967	5	NULL	NULL	0	NULL	5-HT3 receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The best studied members of the Cys-loop family are nACh , 5-HT3 , GABAA and glycine receptors .
	manualset3
142991	4	408967	5	NULL	NULL	0	NULL	GABAA receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The best studied members of the Cys-loop family are nACh , 5-HT3 , GABAA and glycine receptors .
	manualset3
142992	5	408967	5	NULL	NULL	0	NULL	glycine receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The best studied members of the Cys-loop family are nACh , 5-HT3 , GABAA and glycine receptors .
	manualset3
142993	1	408968	5	NULL	NULL	0	NULL	beta-adrenoceptor coronary vasodilatation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The beta-adrenoceptor coronary vasodilatation is an example of feedforward open-loop control that complements the closed-loop negative feedback control by local metabolic factors .
	manualset3
142994	2	408968	5	NULL	NULL	0	NULL	example 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The beta-adrenoceptor coronary vasodilatation is an example of feedforward open-loop control that complements the closed-loop negative feedback control by local metabolic factors .
	manualset3
142995	3	408968	5	NULL	NULL	NULL	NULL	feedforward open-loop control 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The beta-adrenoceptor coronary vasodilatation is an example of feedforward open-loop control that complements the closed-loop negative feedback control by local metabolic factors .
	manualset3
142996	4	408968	5	NULL	NULL	0	NULL	closed-loop negative feedback control	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The beta-adrenoceptor coronary vasodilatation is an example of feedforward open-loop control that complements the closed-loop negative feedback control by local metabolic factors .
	manualset3
142997	5	408968	5	NULL	NULL	0	NULL	local metabolic factors	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The beta-adrenoceptor coronary vasodilatation is an example of feedforward open-loop control that complements the closed-loop negative feedback control by local metabolic factors .
	manualset3
142998	1	408969	5	NULL	NULL	NULL	NULL	group of fasted males 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A separate group of fasted males was refed after 4 h of sampling ; the plasma levels of GH , insulin , and metabolites returned to those observed in birds given feed ad libitum within 30 min of refeeding .
	manualset3
142999	2	408969	5	NULL	NULL	0	NULL	 4 h 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A separate group of fasted males was refed after 4 h of sampling ; the plasma levels of GH , insulin , and metabolites returned to those observed in birds given feed ad libitum within 30 min of refeeding .
	manualset3
143000	3	408969	5	NULL	NULL	0	NULL	sampling 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A separate group of fasted males was refed after 4 h of sampling ; the plasma levels of GH , insulin , and metabolites returned to those observed in birds given feed ad libitum within 30 min of refeeding .
	manualset3
143001	4	408969	5	NULL	NULL	0	NULL	plasma levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A separate group of fasted males was refed after 4 h of sampling ; the plasma levels of GH , insulin , and metabolites returned to those observed in birds given feed ad libitum within 30 min of refeeding .
	manualset3
143002	5	408969	5	NULL	NULL	0	NULL	GH 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A separate group of fasted males was refed after 4 h of sampling ; the plasma levels of GH , insulin , and metabolites returned to those observed in birds given feed ad libitum within 30 min of refeeding .
	manualset3
143003	6	408969	5	NULL	NULL	0	NULL	insulin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A separate group of fasted males was refed after 4 h of sampling ; the plasma levels of GH , insulin , and metabolites returned to those observed in birds given feed ad libitum within 30 min of refeeding .
	manualset3
143004	7	408969	5	NULL	NULL	0	NULL	metabolites 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A separate group of fasted males was refed after 4 h of sampling ; the plasma levels of GH , insulin , and metabolites returned to those observed in birds given feed ad libitum within 30 min of refeeding .
	manualset3
143005	8	408969	5	NULL	NULL	0	NULL	birds 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A separate group of fasted males was refed after 4 h of sampling ; the plasma levels of GH , insulin , and metabolites returned to those observed in birds given feed ad libitum within 30 min of refeeding .
	manualset3
143006	9	408969	5	NULL	NULL	0	NULL	feed 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A separate group of fasted males was refed after 4 h of sampling ; the plasma levels of GH , insulin , and metabolites returned to those observed in birds given feed ad libitum within 30 min of refeeding .
	manualset3
143007	10	408969	5	NULL	NULL	0	NULL	30 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A separate group of fasted males was refed after 4 h of sampling ; the plasma levels of GH , insulin , and metabolites returned to those observed in birds given feed ad libitum within 30 min of refeeding .
	manualset3
143008	1	408970	5	NULL	NULL	0	NULL	beta-amyloid protein ( Abeta ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The beta-amyloid protein ( Abeta ) is the major protein component of amyloid plaques found in the Alzheimer brain .
	manualset3
143009	2	408970	5	NULL	NULL	0	NULL	protein component	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The beta-amyloid protein ( Abeta ) is the major protein component of amyloid plaques found in the Alzheimer brain .
	manualset3
143010	3	408970	5	NULL	NULL	0	NULL	amyloid plaques	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The beta-amyloid protein ( Abeta ) is the major protein component of amyloid plaques found in the Alzheimer brain .
	manualset3
143011	4	408970	5	NULL	NULL	0	NULL	Alzheimer brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The beta-amyloid protein ( Abeta ) is the major protein component of amyloid plaques found in the Alzheimer brain .
	manualset3
143012	1	408971	5	NULL	NULL	NULL	NULL	beta-lactamases 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The beta-lactamases can be divided into four classes ( A , B , C , and D ) , each of which contains both chromosomal and plasmid-encoded enzymes .
	manualset3
143013	2	408971	5	NULL	NULL	0	NULL	four classes ( A , B , C , and D )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The beta-lactamases can be divided into four classes ( A , B , C , and D ) , each of which contains both chromosomal and plasmid-encoded enzymes .
	manualset3
143014	3	408971	5	NULL	NULL	0	NULL	chromosomal enzymes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The beta-lactamases can be divided into four classes ( A , B , C , and D ) , each of which contains both chromosomal and plasmid-encoded enzymes .
	manualset3
143015	4	408971	5	NULL	NULL	0	NULL	plasmid-encoded enzymes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The beta-lactamases can be divided into four classes ( A , B , C , and D ) , each of which contains both chromosomal and plasmid-encoded enzymes .
	manualset3
143016	1	408972	5	NULL	NULL	0	NULL	beta chain 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The beta chain by itself does not bind IL-5 , but it can convert the low affinity IL-5R into the high affinity IL-5R and in indispensable for IL-5 signal transduction .
	manualset3
143017	2	408972	5	NULL	NULL	0	NULL	IL-5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The beta chain by itself does not bind IL-5 , but it can convert the low affinity IL-5R into the high affinity IL-5R and in indispensable for IL-5 signal transduction .
	manualset3
143018	3	408972	5	NULL	NULL	NULL	NULL	low affinity IL-5R	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The beta chain by itself does not bind IL-5 , but it can convert the low affinity IL-5R into the high affinity IL-5R and in indispensable for IL-5 signal transduction .
	manualset3
143019	4	408972	5	NULL	NULL	NULL	NULL	high affinity IL-5R 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The beta chain by itself does not bind IL-5 , but it can convert the low affinity IL-5R into the high affinity IL-5R and in indispensable for IL-5 signal transduction .
	manualset3
143020	5	408972	5	NULL	NULL	0	NULL	IL-5 signal transduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The beta chain by itself does not bind IL-5 , but it can convert the low affinity IL-5R into the high affinity IL-5R and in indispensable for IL-5 signal transduction .
	manualset3
143021	1	408973	5	NULL	NULL	0	NULL	beta chain gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The beta chain gene of T cell receptor rearrangement analysis is necessary for distinguishing of T LGL lymphocytosis from T LGL leukemia .
	manualset3
143022	2	408973	5	NULL	NULL	0	NULL	T cell receptor rearrangement analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The beta chain gene of T cell receptor rearrangement analysis is necessary for distinguishing of T LGL lymphocytosis from T LGL leukemia .
	manualset3
143023	3	408973	5	NULL	NULL	0	NULL	T LGL lymphocytosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The beta chain gene of T cell receptor rearrangement analysis is necessary for distinguishing of T LGL lymphocytosis from T LGL leukemia .
	manualset3
143024	4	408973	5	NULL	NULL	0	NULL	T LGL leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The beta chain gene of T cell receptor rearrangement analysis is necessary for distinguishing of T LGL lymphocytosis from T LGL leukemia .
	manualset3
143025	1	408974	5	NULL	NULL	0	NULL	beta subunit	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The beta subunit and heterodimer specific antibodies inhibited both hormone binding and response , while the alpha subunit specific antibodies inhibited response without affecting binding .
	manualset3
143026	2	408974	5	NULL	NULL	0	NULL	heterodimer specific antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The beta subunit and heterodimer specific antibodies inhibited both hormone binding and response , while the alpha subunit specific antibodies inhibited response without affecting binding .
	manualset3
143027	3	408974	5	NULL	NULL	0	NULL	hormone binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The beta subunit and heterodimer specific antibodies inhibited both hormone binding and response , while the alpha subunit specific antibodies inhibited response without affecting binding .
	manualset3
143028	4	408974	5	NULL	NULL	0	NULL	response 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The beta subunit and heterodimer specific antibodies inhibited both hormone binding and response , while the alpha subunit specific antibodies inhibited response without affecting binding .
	manualset3
143029	5	408974	5	NULL	NULL	0	NULL	alpha subunit specific antibodies 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The beta subunit and heterodimer specific antibodies inhibited both hormone binding and response , while the alpha subunit specific antibodies inhibited response without affecting binding .
	manualset3
143030	6	408974	5	NULL	NULL	0	NULL	response 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The beta subunit and heterodimer specific antibodies inhibited both hormone binding and response , while the alpha subunit specific antibodies inhibited response without affecting binding .
	manualset3
143031	7	408974	5	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The beta subunit and heterodimer specific antibodies inhibited both hormone binding and response , while the alpha subunit specific antibodies inhibited response without affecting binding .
	manualset3
143032	1	408975	5	NULL	NULL	0	NULL	beta2-m creatinine index	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The beta2-m creatinine index of random urine samples was 23.5 + / - 16.6 microg/g ( n = 26 ) .
	manualset3
143033	2	408975	5	NULL	NULL	0	NULL	random urine samples	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The beta2-m creatinine index of random urine samples was 23.5 + / - 16.6 microg/g ( n = 26 ) .
	manualset3
143034	3	408975	5	NULL	NULL	0	NULL	 23.5 + / - 16.6 microg/g ( n = 26 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The beta2-m creatinine index of random urine samples was 23.5 + / - 16.6 microg/g ( n = 26 ) .
	manualset3
143035	1	408976	5	NULL	NULL	0	NULL	bi-modal maximum	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The bi-modal maximum indicates the influence of two intermediate metabolites in spectinomycin biosynthesis .
	manualset3
143036	2	408976	5	NULL	NULL	0	NULL	influence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The bi-modal maximum indicates the influence of two intermediate metabolites in spectinomycin biosynthesis .
	manualset3
143037	3	408976	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The bi-modal maximum indicates the influence of two intermediate metabolites in spectinomycin biosynthesis .
	manualset3
143038	4	408976	5	NULL	NULL	0	NULL	intermediate metabolites	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The bi-modal maximum indicates the influence of two intermediate metabolites in spectinomycin biosynthesis .
	manualset3
143039	5	408976	5	NULL	NULL	0	NULL	spectinomycin biosynthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The bi-modal maximum indicates the influence of two intermediate metabolites in spectinomycin biosynthesis .
	manualset3
143040	1	408977	5	NULL	NULL	0	NULL	bile ducts 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The bile ducts were dilated on sonography in 26 patients .
	manualset3
143041	2	408977	5	NULL	NULL	0	NULL	sonography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The bile ducts were dilated on sonography in 26 patients .
	manualset3
143042	3	408977	5	NULL	NULL	NULL	NULL	26	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The bile ducts were dilated on sonography in 26 patients .
	manualset3
143043	4	408977	5	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The bile ducts were dilated on sonography in 26 patients .
	manualset3
143044	1	408978	5	NULL	NULL	0	NULL	bile metabolic profile	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The bile metabolic profile of O. bonariensis was characterized by some abundant metabolite ions corresponding with taurine conjugated bile acids , which were useful as reference peaks .
	manualset3
143045	2	408978	5	NULL	NULL	0	NULL	O. bonariensis 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The bile metabolic profile of O. bonariensis was characterized by some abundant metabolite ions corresponding with taurine conjugated bile acids , which were useful as reference peaks .
	manualset3
143046	3	408978	5	NULL	NULL	0	NULL	metabolite ions 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The bile metabolic profile of O. bonariensis was characterized by some abundant metabolite ions corresponding with taurine conjugated bile acids , which were useful as reference peaks .
	manualset3
143047	4	408978	5	NULL	NULL	0	NULL	taurine conjugated bile acids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The bile metabolic profile of O. bonariensis was characterized by some abundant metabolite ions corresponding with taurine conjugated bile acids , which were useful as reference peaks .
	manualset3
143048	5	408978	5	NULL	NULL	0	NULL	reference peaks	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The bile metabolic profile of O. bonariensis was characterized by some abundant metabolite ions corresponding with taurine conjugated bile acids , which were useful as reference peaks .
	manualset3
143049	1	408979	5	NULL	NULL	0	NULL	biliary CTRX levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The biliary CTRX levels increased rapidly and were sustained as high as 92.5-219 micrograms/ml in all patients even 24 hours after 2 g of CTRX was infused intravenously once daily .
	manualset3
143050	2	408979	5	NULL	NULL	0	NULL	92.5-219 micrograms/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The biliary CTRX levels increased rapidly and were sustained as high as 92.5-219 micrograms/ml in all patients even 24 hours after 2 g of CTRX was infused intravenously once daily .
	manualset3
143051	3	408979	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The biliary CTRX levels increased rapidly and were sustained as high as 92.5-219 micrograms/ml in all patients even 24 hours after 2 g of CTRX was infused intravenously once daily .
	manualset3
143052	4	408979	5	NULL	NULL	0	NULL	24 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The biliary CTRX levels increased rapidly and were sustained as high as 92.5-219 micrograms/ml in all patients even 24 hours after 2 g of CTRX was infused intravenously once daily .
	manualset3
143053	5	408979	5	NULL	NULL	0	NULL	2 g 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The biliary CTRX levels increased rapidly and were sustained as high as 92.5-219 micrograms/ml in all patients even 24 hours after 2 g of CTRX was infused intravenously once daily .
	manualset3
143054	6	408979	5	NULL	NULL	0	NULL	CTRX 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The biliary CTRX levels increased rapidly and were sustained as high as 92.5-219 micrograms/ml in all patients even 24 hours after 2 g of CTRX was infused intravenously once daily .
	manualset3
143055	1	408980	5	NULL	NULL	0	NULL	HSP70 promoter deletion constructs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of HSP70 promoter deletion constructs was established .
	manualset3
143056	1	408981	5	NULL	NULL	0	NULL	binding affinity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding affinity is strongly reduced ( more than 14.5 kJ/mol ) if a cAMP derivative is no longer able to form a hydrogen bond at N6H2 , or at O3 ' .
	manualset3
143057	2	408981	5	NULL	NULL	0	NULL	14.5 kJ/mol	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding affinity is strongly reduced ( more than 14.5 kJ/mol ) if a cAMP derivative is no longer able to form a hydrogen bond at N6H2 , or at O3 ' .
	manualset3
143058	3	408981	5	NULL	NULL	0	NULL	cAMP derivative	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding affinity is strongly reduced ( more than 14.5 kJ/mol ) if a cAMP derivative is no longer able to form a hydrogen bond at N6H2 , or at O3 ' .
	manualset3
143059	4	408981	5	NULL	NULL	0	NULL	hydrogen bond	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding affinity is strongly reduced ( more than 14.5 kJ/mol ) if a cAMP derivative is no longer able to form a hydrogen bond at N6H2 , or at O3 ' .
	manualset3
143060	5	408981	5	NULL	NULL	0	NULL	N6H2 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding affinity is strongly reduced ( more than 14.5 kJ/mol ) if a cAMP derivative is no longer able to form a hydrogen bond at N6H2 , or at O3 ' .
	manualset3
143061	6	408981	5	NULL	NULL	0	NULL	O3 ' 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding affinity is strongly reduced ( more than 14.5 kJ/mol ) if a cAMP derivative is no longer able to form a hydrogen bond at N6H2 , or at O3 ' .
	manualset3
143062	1	408982	5	NULL	NULL	0	NULL	binding affinity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding affinity of one of the two peptides could be increased by appropriate substitutions of the anchor residues with those of the known HLA-A3 anchor motifs .
	manualset3
143063	2	408982	5	NULL	NULL	0	NULL	one of the two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding affinity of one of the two peptides could be increased by appropriate substitutions of the anchor residues with those of the known HLA-A3 anchor motifs .
	manualset3
143064	3	408982	5	NULL	NULL	0	NULL	peptides 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding affinity of one of the two peptides could be increased by appropriate substitutions of the anchor residues with those of the known HLA-A3 anchor motifs .
	manualset3
143065	4	408982	5	NULL	NULL	0	NULL	substitutions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding affinity of one of the two peptides could be increased by appropriate substitutions of the anchor residues with those of the known HLA-A3 anchor motifs .
	manualset3
143066	5	408982	5	NULL	NULL	NULL	NULL	anchor residues	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The binding affinity of one of the two peptides could be increased by appropriate substitutions of the anchor residues with those of the known HLA-A3 anchor motifs .
	manualset3
143067	6	408982	5	NULL	NULL	0	NULL	HLA-A3 anchor motifs 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding affinity of one of the two peptides could be increased by appropriate substitutions of the anchor residues with those of the known HLA-A3 anchor motifs .
	manualset3
143068	1	408983	5	NULL	NULL	0	NULL	binding affinity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding affinity of the recombinant PpPPR_71 was strongest when using the edited RNA at ccmF-1 .
	manualset3
143069	2	408983	5	NULL	NULL	0	NULL	recombinant PpPPR_71	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding affinity of the recombinant PpPPR_71 was strongest when using the edited RNA at ccmF-1 .
	manualset3
143070	3	408983	5	NULL	NULL	0	NULL	edited RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding affinity of the recombinant PpPPR_71 was strongest when using the edited RNA at ccmF-1 .
	manualset3
143071	4	408983	5	NULL	NULL	0	NULL	ccmF-1	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding affinity of the recombinant PpPPR_71 was strongest when using the edited RNA at ccmF-1 .
	manualset3
143072	1	408984	5	NULL	NULL	0	NULL	binding behavior	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding behavior toward DNA of some minor groove binders related to distamycin was studied by means of circular dichroism .
	manualset3
143073	2	408984	5	NULL	NULL	0	NULL	DNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding behavior toward DNA of some minor groove binders related to distamycin was studied by means of circular dichroism .
	manualset3
143074	3	408984	5	NULL	NULL	0	NULL	minor groove binders 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding behavior toward DNA of some minor groove binders related to distamycin was studied by means of circular dichroism .
	manualset3
143075	4	408984	5	NULL	NULL	0	NULL	distamycin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding behavior toward DNA of some minor groove binders related to distamycin was studied by means of circular dichroism .
	manualset3
143076	5	408984	5	NULL	NULL	0	NULL	circular dichroism	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding behavior toward DNA of some minor groove binders related to distamycin was studied by means of circular dichroism .
	manualset3
143077	1	408985	5	NULL	NULL	0	NULL	binding characteristics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding characteristics analyzed for HC homogenates and retinal homogenates revealed that ( 3H ) PDBu binding is time dependent , specific , saturable , and reversible .
	manualset3
143078	2	408985	5	NULL	NULL	0	NULL	HC homogenates	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding characteristics analyzed for HC homogenates and retinal homogenates revealed that ( 3H ) PDBu binding is time dependent , specific , saturable , and reversible .
	manualset3
143079	3	408985	5	NULL	NULL	0	NULL	retinal homogenates 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding characteristics analyzed for HC homogenates and retinal homogenates revealed that ( 3H ) PDBu binding is time dependent , specific , saturable , and reversible .
	manualset3
143080	4	408985	5	NULL	NULL	0	NULL	( 3H ) PDBu binding  	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding characteristics analyzed for HC homogenates and retinal homogenates revealed that ( 3H ) PDBu binding is time dependent , specific , saturable , and reversible .
	manualset3
143081	5	408985	5	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding characteristics analyzed for HC homogenates and retinal homogenates revealed that ( 3H ) PDBu binding is time dependent , specific , saturable , and reversible .
	manualset3
143082	1	408986	5	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of ( 125I ) T4 to serum proteins was studied in human , monkey , cattle , sheep , goat , water buffalo , horse , swine , dog , cat , rabbit , rat , chicken , frog , and salmon .
	manualset3
143083	2	408986	5	NULL	NULL	0	NULL	 ( 125I ) T4	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of ( 125I ) T4 to serum proteins was studied in human , monkey , cattle , sheep , goat , water buffalo , horse , swine , dog , cat , rabbit , rat , chicken , frog , and salmon .
	manualset3
143084	3	408986	5	NULL	NULL	0	NULL	serum proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of ( 125I ) T4 to serum proteins was studied in human , monkey , cattle , sheep , goat , water buffalo , horse , swine , dog , cat , rabbit , rat , chicken , frog , and salmon .
	manualset3
143085	4	408986	5	NULL	NULL	0	NULL	human 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of ( 125I ) T4 to serum proteins was studied in human , monkey , cattle , sheep , goat , water buffalo , horse , swine , dog , cat , rabbit , rat , chicken , frog , and salmon .
	manualset3
143086	5	408986	5	NULL	NULL	0	NULL	monkey 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of ( 125I ) T4 to serum proteins was studied in human , monkey , cattle , sheep , goat , water buffalo , horse , swine , dog , cat , rabbit , rat , chicken , frog , and salmon .
	manualset3
143087	6	408986	5	NULL	NULL	0	NULL	cattle 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of ( 125I ) T4 to serum proteins was studied in human , monkey , cattle , sheep , goat , water buffalo , horse , swine , dog , cat , rabbit , rat , chicken , frog , and salmon .
	manualset3
143088	7	408986	5	NULL	NULL	0	NULL	sheep 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of ( 125I ) T4 to serum proteins was studied in human , monkey , cattle , sheep , goat , water buffalo , horse , swine , dog , cat , rabbit , rat , chicken , frog , and salmon .
	manualset3
143089	8	408986	5	NULL	NULL	0	NULL	goat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of ( 125I ) T4 to serum proteins was studied in human , monkey , cattle , sheep , goat , water buffalo , horse , swine , dog , cat , rabbit , rat , chicken , frog , and salmon .
	manualset3
143090	9	408986	5	NULL	NULL	0	NULL	water buffalo	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of ( 125I ) T4 to serum proteins was studied in human , monkey , cattle , sheep , goat , water buffalo , horse , swine , dog , cat , rabbit , rat , chicken , frog , and salmon .
	manualset3
143091	10	408986	5	NULL	NULL	0	NULL	horse 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of ( 125I ) T4 to serum proteins was studied in human , monkey , cattle , sheep , goat , water buffalo , horse , swine , dog , cat , rabbit , rat , chicken , frog , and salmon .
	manualset3
143092	11	408986	5	NULL	NULL	0	NULL	swine 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of ( 125I ) T4 to serum proteins was studied in human , monkey , cattle , sheep , goat , water buffalo , horse , swine , dog , cat , rabbit , rat , chicken , frog , and salmon .
	manualset3
143093	12	408986	5	NULL	NULL	0	NULL	dog 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of ( 125I ) T4 to serum proteins was studied in human , monkey , cattle , sheep , goat , water buffalo , horse , swine , dog , cat , rabbit , rat , chicken , frog , and salmon .
	manualset3
143094	13	408986	5	NULL	NULL	0	NULL	cat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of ( 125I ) T4 to serum proteins was studied in human , monkey , cattle , sheep , goat , water buffalo , horse , swine , dog , cat , rabbit , rat , chicken , frog , and salmon .
	manualset3
143095	14	408986	5	NULL	NULL	0	NULL	rabbit 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of ( 125I ) T4 to serum proteins was studied in human , monkey , cattle , sheep , goat , water buffalo , horse , swine , dog , cat , rabbit , rat , chicken , frog , and salmon .
	manualset3
143096	15	408986	5	NULL	NULL	0	NULL	rat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of ( 125I ) T4 to serum proteins was studied in human , monkey , cattle , sheep , goat , water buffalo , horse , swine , dog , cat , rabbit , rat , chicken , frog , and salmon .
	manualset3
143097	16	408986	5	NULL	NULL	0	NULL	chicken 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of ( 125I ) T4 to serum proteins was studied in human , monkey , cattle , sheep , goat , water buffalo , horse , swine , dog , cat , rabbit , rat , chicken , frog , and salmon .
	manualset3
143098	17	408986	5	NULL	NULL	0	NULL	frog 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of ( 125I ) T4 to serum proteins was studied in human , monkey , cattle , sheep , goat , water buffalo , horse , swine , dog , cat , rabbit , rat , chicken , frog , and salmon .
	manualset3
143099	18	408986	5	NULL	NULL	0	NULL	salmon 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of ( 125I ) T4 to serum proteins was studied in human , monkey , cattle , sheep , goat , water buffalo , horse , swine , dog , cat , rabbit , rat , chicken , frog , and salmon .
	manualset3
143100	1	408987	5	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of F14 .6 to lymphocytes and Chinese hamster ovary cells was inhibited by soluble CRT or SPA-600 .
	manualset3
143101	2	408987	5	NULL	NULL	0	NULL	F14.6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of F14 .6 to lymphocytes and Chinese hamster ovary cells was inhibited by soluble CRT or SPA-600 .
	manualset3
143102	3	408987	5	NULL	NULL	0	NULL	lymphocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of F14 .6 to lymphocytes and Chinese hamster ovary cells was inhibited by soluble CRT or SPA-600 .
	manualset3
143103	4	408987	5	NULL	NULL	0	NULL	Chinese hamster ovary cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of F14 .6 to lymphocytes and Chinese hamster ovary cells was inhibited by soluble CRT or SPA-600 .
	manualset3
143104	5	408987	5	NULL	NULL	0	NULL	soluble CRT 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of F14 .6 to lymphocytes and Chinese hamster ovary cells was inhibited by soluble CRT or SPA-600 .
	manualset3
143105	6	408987	5	NULL	NULL	0	NULL	SPA-600	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of F14 .6 to lymphocytes and Chinese hamster ovary cells was inhibited by soluble CRT or SPA-600 .
	manualset3
143106	1	408988	5	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of antigens with antibodies forms immune complexes in the body .
	manualset3
143107	2	408988	5	NULL	NULL	0	NULL	antigens 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of antigens with antibodies forms immune complexes in the body .
	manualset3
143108	3	408988	5	NULL	NULL	0	NULL	antibodies 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of antigens with antibodies forms immune complexes in the body .
	manualset3
143109	4	408988	5	NULL	NULL	0	NULL	immune complexes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of antigens with antibodies forms immune complexes in the body .
	manualset3
143110	5	408988	5	NULL	NULL	0	NULL	body 	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of antigens with antibodies forms immune complexes in the body .
	manualset3
143111	1	408989	5	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of antinuclear antibody-positive juvenile arthritis ( JA ) sera to bovine thymus histones H1 , H2A , H2B , H3 , and H4 was studied by an enzyme-linked immunosorbent assay .
	manualset3
143112	2	408989	5	NULL	NULL	0	NULL	antinuclear antibody-positive juvenile arthritis ( JA ) sera	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of antinuclear antibody-positive juvenile arthritis ( JA ) sera to bovine thymus histones H1 , H2A , H2B , H3 , and H4 was studied by an enzyme-linked immunosorbent assay .
	manualset3
143113	3	408989	5	NULL	NULL	0	NULL	bovine thymus histones H1	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of antinuclear antibody-positive juvenile arthritis ( JA ) sera to bovine thymus histones H1 , H2A , H2B , H3 , and H4 was studied by an enzyme-linked immunosorbent assay .
	manualset3
143114	4	408989	5	NULL	NULL	0	NULL	bovine thymus histones H2A	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of antinuclear antibody-positive juvenile arthritis ( JA ) sera to bovine thymus histones H1 , H2A , H2B , H3 , and H4 was studied by an enzyme-linked immunosorbent assay .
	manualset3
143115	5	408989	5	NULL	NULL	0	NULL	bovine thymus histones H2B	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of antinuclear antibody-positive juvenile arthritis ( JA ) sera to bovine thymus histones H1 , H2A , H2B , H3 , and H4 was studied by an enzyme-linked immunosorbent assay .
	manualset3
143116	6	408989	5	NULL	NULL	0	NULL	bovine thymus histones H3	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of antinuclear antibody-positive juvenile arthritis ( JA ) sera to bovine thymus histones H1 , H2A , H2B , H3 , and H4 was studied by an enzyme-linked immunosorbent assay .
	manualset3
143117	7	408989	5	NULL	NULL	0	NULL	bovine thymus histones H4	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of antinuclear antibody-positive juvenile arthritis ( JA ) sera to bovine thymus histones H1 , H2A , H2B , H3 , and H4 was studied by an enzyme-linked immunosorbent assay .
	manualset3
143118	8	408989	5	NULL	NULL	0	NULL	enzyme-linked immunosorbent assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of antinuclear antibody-positive juvenile arthritis ( JA ) sera to bovine thymus histones H1 , H2A , H2B , H3 , and H4 was studied by an enzyme-linked immunosorbent assay .
	manualset3
143119	1	408990	5	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of approximately 5 mol of spermine/mol of nardilysin was demonstrated .
	manualset3
143120	2	408990	5	NULL	NULL	0	NULL	5 mol of spermine/mol of nardilysin	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of approximately 5 mol of spermine/mol of nardilysin was demonstrated .
	manualset3
143121	1	408991	5	NULL	NULL	0	NULL	series 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of N-methyl-bisindolylmaleimide derivatives was synthesized and evaluated as cell death inhibitors .
	manualset3
143122	2	408991	5	NULL	NULL	0	NULL	 N-methyl-bisindolylmaleimide derivatives	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of N-methyl-bisindolylmaleimide derivatives was synthesized and evaluated as cell death inhibitors .
	manualset3
143123	3	408991	5	NULL	NULL	0	NULL	cell death inhibitors	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of N-methyl-bisindolylmaleimide derivatives was synthesized and evaluated as cell death inhibitors .
	manualset3
143124	1	408992	5	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of ligands can reduce significantly , or even overwhelm , its effects .
	manualset3
143125	2	408992	5	NULL	NULL	0	NULL	ligands 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of ligands can reduce significantly , or even overwhelm , its effects .
	manualset3
143126	3	408992	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of ligands can reduce significantly , or even overwhelm , its effects .
	manualset3
143127	1	408993	5	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of reduced cello-dextrins to cellulose required at least 4 consecutive 1 , 4-beta-glucosyl residues .
	manualset3
143128	2	408993	5	NULL	NULL	0	NULL	cello-dextrins	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of reduced cello-dextrins to cellulose required at least 4 consecutive 1 , 4-beta-glucosyl residues .
	manualset3
143129	3	408993	5	NULL	NULL	0	NULL	cellulose 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of reduced cello-dextrins to cellulose required at least 4 consecutive 1 , 4-beta-glucosyl residues .
	manualset3
143130	4	408993	5	NULL	NULL	0	NULL	4 consecutive 1 , 4-beta-glucosyl residues	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding of reduced cello-dextrins to cellulose required at least 4 consecutive 1 , 4-beta-glucosyl residues .
	manualset3
143131	1	408994	5	NULL	NULL	0	NULL	binding parameters	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding parameters of N-acetyl-D-galactosamine and methyl-N-acetyl-alpha-D - galactosaminide , were determined by titrating the perturbation in the absorption spectrum of the protein .
	manualset3
143132	2	408994	5	NULL	NULL	0	NULL	N-acetyl-D-galactosamine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding parameters of N-acetyl-D-galactosamine and methyl-N-acetyl-alpha-D - galactosaminide , were determined by titrating the perturbation in the absorption spectrum of the protein .
	manualset3
143133	3	408994	5	NULL	NULL	0	NULL	methyl-N-acetyl-alpha-D - galactosaminide	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding parameters of N-acetyl-D-galactosamine and methyl-N-acetyl-alpha-D - galactosaminide , were determined by titrating the perturbation in the absorption spectrum of the protein .
	manualset3
143134	4	408994	5	NULL	NULL	0	NULL	perturbation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding parameters of N-acetyl-D-galactosamine and methyl-N-acetyl-alpha-D - galactosaminide , were determined by titrating the perturbation in the absorption spectrum of the protein .
	manualset3
143135	5	408994	5	NULL	NULL	0	NULL	absorption spectrum	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding parameters of N-acetyl-D-galactosamine and methyl-N-acetyl-alpha-D - galactosaminide , were determined by titrating the perturbation in the absorption spectrum of the protein .
	manualset3
143136	6	408994	5	NULL	NULL	0	NULL	protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding parameters of N-acetyl-D-galactosamine and methyl-N-acetyl-alpha-D - galactosaminide , were determined by titrating the perturbation in the absorption spectrum of the protein .
	manualset3
143137	1	408995	5	NULL	NULL	0	NULL	binding polarity	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding polarity onto hsp27pal is accompanied by different contribution of the UspDBD and EcRDBD C-terminal sequences to the DNA-binding and heterocomplex formation .
	manualset3
143138	2	408995	5	NULL	NULL	0	NULL	hsp27pal 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding polarity onto hsp27pal is accompanied by different contribution of the UspDBD and EcRDBD C-terminal sequences to the DNA-binding and heterocomplex formation .
	manualset3
143139	3	408995	5	NULL	NULL	0	NULL	contribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding polarity onto hsp27pal is accompanied by different contribution of the UspDBD and EcRDBD C-terminal sequences to the DNA-binding and heterocomplex formation .
	manualset3
143140	4	408995	5	NULL	NULL	NULL	NULL	UspDBD C-terminal sequence	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The binding polarity onto hsp27pal is accompanied by different contribution of the UspDBD and EcRDBD C-terminal sequences to the DNA-binding and heterocomplex formation .
	manualset3
143141	5	408995	5	NULL	NULL	NULL	NULL	EcRDBD C-terminal sequence	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The binding polarity onto hsp27pal is accompanied by different contribution of the UspDBD and EcRDBD C-terminal sequences to the DNA-binding and heterocomplex formation .
	manualset3
143142	6	408995	5	NULL	NULL	0	NULL	DNA-binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding polarity onto hsp27pal is accompanied by different contribution of the UspDBD and EcRDBD C-terminal sequences to the DNA-binding and heterocomplex formation .
	manualset3
143143	7	408995	5	NULL	NULL	0	NULL	heterocomplex formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding polarity onto hsp27pal is accompanied by different contribution of the UspDBD and EcRDBD C-terminal sequences to the DNA-binding and heterocomplex formation .
	manualset3
143144	1	408996	5	NULL	NULL	0	NULL	binding profiles	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding profiles obtained in these areas were clearly distinct from those obtained in the CA1 layer of the hippocampus and in the pontine nuclei , regions enriched in M1 and M2 sites , respectively .
	manualset3
143145	2	408996	5	NULL	NULL	0	NULL	areas 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding profiles obtained in these areas were clearly distinct from those obtained in the CA1 layer of the hippocampus and in the pontine nuclei , regions enriched in M1 and M2 sites , respectively .
	manualset3
143146	3	408996	5	NULL	NULL	0	NULL	CA1 layer of the hippocampus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding profiles obtained in these areas were clearly distinct from those obtained in the CA1 layer of the hippocampus and in the pontine nuclei , regions enriched in M1 and M2 sites , respectively .
	manualset3
143147	4	408996	5	NULL	NULL	0	NULL	pontine nuclei 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding profiles obtained in these areas were clearly distinct from those obtained in the CA1 layer of the hippocampus and in the pontine nuclei , regions enriched in M1 and M2 sites , respectively .
	manualset3
143148	5	408996	5	NULL	NULL	0	NULL	regions enriched in M1 sites	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding profiles obtained in these areas were clearly distinct from those obtained in the CA1 layer of the hippocampus and in the pontine nuclei , regions enriched in M1 and M2 sites , respectively .
	manualset3
143149	6	408996	5	NULL	NULL	0	NULL	regions enriched in M2 sites	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding profiles obtained in these areas were clearly distinct from those obtained in the CA1 layer of the hippocampus and in the pontine nuclei , regions enriched in M1 and M2 sites , respectively .
	manualset3
143150	1	408997	5	NULL	NULL	0	NULL	binding specificity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding specificity of the VLDLR and LDLR for apoC1-enriched lipoprotein particles was examined in vivo through adenovirus-mediated gene transfer of the VLDLR and the LDLR ( giving rise to adenovirus-containing ( Ad ) - VLDLR and Ad-LDLR respectively ) in APOC1 transgenic mice , LDLR-deficient ( LDLR - / - ) mice and wild-type mice .
	manualset3
143151	2	408997	5	NULL	NULL	0	NULL	VLDLR 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding specificity of the VLDLR and LDLR for apoC1-enriched lipoprotein particles was examined in vivo through adenovirus-mediated gene transfer of the VLDLR and the LDLR ( giving rise to adenovirus-containing ( Ad ) - VLDLR and Ad-LDLR respectively ) in APOC1 transgenic mice , LDLR-deficient ( LDLR - / - ) mice and wild-type mice .
	manualset3
143152	3	408997	5	NULL	NULL	0	NULL	LDLR 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding specificity of the VLDLR and LDLR for apoC1-enriched lipoprotein particles was examined in vivo through adenovirus-mediated gene transfer of the VLDLR and the LDLR ( giving rise to adenovirus-containing ( Ad ) - VLDLR and Ad-LDLR respectively ) in APOC1 transgenic mice , LDLR-deficient ( LDLR - / - ) mice and wild-type mice .
	manualset3
143153	4	408997	5	NULL	NULL	0	NULL	apoC1-enriched lipoprotein particles 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding specificity of the VLDLR and LDLR for apoC1-enriched lipoprotein particles was examined in vivo through adenovirus-mediated gene transfer of the VLDLR and the LDLR ( giving rise to adenovirus-containing ( Ad ) - VLDLR and Ad-LDLR respectively ) in APOC1 transgenic mice , LDLR-deficient ( LDLR - / - ) mice and wild-type mice .
	manualset3
143154	5	408997	5	NULL	NULL	0	NULL	adenovirus-mediated gene transfer	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding specificity of the VLDLR and LDLR for apoC1-enriched lipoprotein particles was examined in vivo through adenovirus-mediated gene transfer of the VLDLR and the LDLR ( giving rise to adenovirus-containing ( Ad ) - VLDLR and Ad-LDLR respectively ) in APOC1 transgenic mice , LDLR-deficient ( LDLR - / - ) mice and wild-type mice .
	manualset3
143155	6	408997	5	NULL	NULL	0	NULL	VLDLR 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding specificity of the VLDLR and LDLR for apoC1-enriched lipoprotein particles was examined in vivo through adenovirus-mediated gene transfer of the VLDLR and the LDLR ( giving rise to adenovirus-containing ( Ad ) - VLDLR and Ad-LDLR respectively ) in APOC1 transgenic mice , LDLR-deficient ( LDLR - / - ) mice and wild-type mice .
	manualset3
143156	7	408997	5	NULL	NULL	0	NULL	LDLR 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding specificity of the VLDLR and LDLR for apoC1-enriched lipoprotein particles was examined in vivo through adenovirus-mediated gene transfer of the VLDLR and the LDLR ( giving rise to adenovirus-containing ( Ad ) - VLDLR and Ad-LDLR respectively ) in APOC1 transgenic mice , LDLR-deficient ( LDLR - / - ) mice and wild-type mice .
	manualset3
143157	8	408997	5	NULL	NULL	0	NULL	adenovirus-containing ( Ad ) - VLDLR	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding specificity of the VLDLR and LDLR for apoC1-enriched lipoprotein particles was examined in vivo through adenovirus-mediated gene transfer of the VLDLR and the LDLR ( giving rise to adenovirus-containing ( Ad ) - VLDLR and Ad-LDLR respectively ) in APOC1 transgenic mice , LDLR-deficient ( LDLR - / - ) mice and wild-type mice .
	manualset3
143158	9	408997	5	NULL	NULL	0	NULL	 Ad-LDLR	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding specificity of the VLDLR and LDLR for apoC1-enriched lipoprotein particles was examined in vivo through adenovirus-mediated gene transfer of the VLDLR and the LDLR ( giving rise to adenovirus-containing ( Ad ) - VLDLR and Ad-LDLR respectively ) in APOC1 transgenic mice , LDLR-deficient ( LDLR - / - ) mice and wild-type mice .
	manualset3
143159	10	408997	5	NULL	NULL	0	NULL	APOC1 transgenic mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding specificity of the VLDLR and LDLR for apoC1-enriched lipoprotein particles was examined in vivo through adenovirus-mediated gene transfer of the VLDLR and the LDLR ( giving rise to adenovirus-containing ( Ad ) - VLDLR and Ad-LDLR respectively ) in APOC1 transgenic mice , LDLR-deficient ( LDLR - / - ) mice and wild-type mice .
	manualset3
143160	11	408997	5	NULL	NULL	0	NULL	LDLR-deficient ( LDLR - / - ) mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding specificity of the VLDLR and LDLR for apoC1-enriched lipoprotein particles was examined in vivo through adenovirus-mediated gene transfer of the VLDLR and the LDLR ( giving rise to adenovirus-containing ( Ad ) - VLDLR and Ad-LDLR respectively ) in APOC1 transgenic mice , LDLR-deficient ( LDLR - / - ) mice and wild-type mice .
	manualset3
143161	12	408997	5	NULL	NULL	0	NULL	wild-type mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding specificity of the VLDLR and LDLR for apoC1-enriched lipoprotein particles was examined in vivo through adenovirus-mediated gene transfer of the VLDLR and the LDLR ( giving rise to adenovirus-containing ( Ad ) - VLDLR and Ad-LDLR respectively ) in APOC1 transgenic mice , LDLR-deficient ( LDLR - / - ) mice and wild-type mice .
	manualset3
143162	1	408998	5	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding was well described by a surface partitioning equilibrium using an effective charge of the peptide of z ( P ) approximately 5.1 + / - 0.5 .
	manualset3
143163	2	408998	5	NULL	NULL	0	NULL	surface partitioning equilibrium	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding was well described by a surface partitioning equilibrium using an effective charge of the peptide of z ( P ) approximately 5.1 + / - 0.5 .
	manualset3
143164	3	408998	5	NULL	NULL	0	NULL	charge 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding was well described by a surface partitioning equilibrium using an effective charge of the peptide of z ( P ) approximately 5.1 + / - 0.5 .
	manualset3
143165	4	408998	5	NULL	NULL	0	NULL	peptide of z ( P ) 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding was well described by a surface partitioning equilibrium using an effective charge of the peptide of z ( P ) approximately 5.1 + / - 0.5 .
	manualset3
143166	5	408998	5	NULL	NULL	0	NULL	5.1 + / - 0.5 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding was well described by a surface partitioning equilibrium using an effective charge of the peptide of z ( P ) approximately 5.1 + / - 0.5 .
	manualset3
143167	1	408999	5	NULL	NULL	0	NULL	binding constant 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding constant of HlyA for glycophorin was estimated , in RBC at sublytic HlyA concentrations , to be 1.5 x 10 ( -9 ) m .
	manualset3
143168	2	408999	5	NULL	NULL	0	NULL	HlyA 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding constant of HlyA for glycophorin was estimated , in RBC at sublytic HlyA concentrations , to be 1.5 x 10 ( -9 ) m .
	manualset3
143169	3	408999	5	NULL	NULL	0	NULL	glycophorin 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding constant of HlyA for glycophorin was estimated , in RBC at sublytic HlyA concentrations , to be 1.5 x 10 ( -9 ) m .
	manualset3
143170	4	408999	5	NULL	NULL	0	NULL	RBC 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding constant of HlyA for glycophorin was estimated , in RBC at sublytic HlyA concentrations , to be 1.5 x 10 ( -9 ) m .
	manualset3
143171	5	408999	5	NULL	NULL	0	NULL	sublytic HlyA concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding constant of HlyA for glycophorin was estimated , in RBC at sublytic HlyA concentrations , to be 1.5 x 10 ( -9 ) m .
	manualset3
143172	6	408999	5	NULL	NULL	0	NULL	1.5 x 10 ( -9 ) m	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding constant of HlyA for glycophorin was estimated , in RBC at sublytic HlyA concentrations , to be 1.5 x 10 ( -9 ) m .
	manualset3
143173	1	409000	5	NULL	NULL	0	NULL	binding protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding protein shifted the ( 32P ) hsp27 EcRE band on a gel mobility shift assay ; formation of the complex with hsp27 EcRE required KCl ( optimal concentration was approximately 75 mM ) .
	manualset3
143174	2	409000	5	NULL	NULL	0	NULL	( 32P ) hsp27 EcRE band 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding protein shifted the ( 32P ) hsp27 EcRE band on a gel mobility shift assay ; formation of the complex with hsp27 EcRE required KCl ( optimal concentration was approximately 75 mM ) .
	manualset3
143175	3	409000	5	NULL	NULL	0	NULL	gel mobility shift assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding protein shifted the ( 32P ) hsp27 EcRE band on a gel mobility shift assay ; formation of the complex with hsp27 EcRE required KCl ( optimal concentration was approximately 75 mM ) .
	manualset3
143176	4	409000	5	NULL	NULL	0	NULL	formation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding protein shifted the ( 32P ) hsp27 EcRE band on a gel mobility shift assay ; formation of the complex with hsp27 EcRE required KCl ( optimal concentration was approximately 75 mM ) .
	manualset3
143177	5	409000	5	NULL	NULL	0	NULL	complex 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding protein shifted the ( 32P ) hsp27 EcRE band on a gel mobility shift assay ; formation of the complex with hsp27 EcRE required KCl ( optimal concentration was approximately 75 mM ) .
	manualset3
143178	6	409000	5	NULL	NULL	0	NULL	hsp27 EcRE	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding protein shifted the ( 32P ) hsp27 EcRE band on a gel mobility shift assay ; formation of the complex with hsp27 EcRE required KCl ( optimal concentration was approximately 75 mM ) .
	manualset3
143179	7	409000	5	NULL	NULL	0	NULL	KCl 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding protein shifted the ( 32P ) hsp27 EcRE band on a gel mobility shift assay ; formation of the complex with hsp27 EcRE required KCl ( optimal concentration was approximately 75 mM ) .
	manualset3
143180	8	409000	5	NULL	NULL	0	NULL	optimal concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding protein shifted the ( 32P ) hsp27 EcRE band on a gel mobility shift assay ; formation of the complex with hsp27 EcRE required KCl ( optimal concentration was approximately 75 mM ) .
	manualset3
143181	9	409000	5	NULL	NULL	0	NULL	75 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding protein shifted the ( 32P ) hsp27 EcRE band on a gel mobility shift assay ; formation of the complex with hsp27 EcRE required KCl ( optimal concentration was approximately 75 mM ) .
	manualset3
143182	1	409001	5	NULL	NULL	0	NULL	Chromosomal research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Chromosomal research in Lund gives new methods for diagnosis and therapy in cancer ) .
	manualset3
143183	2	409001	5	NULL	NULL	0	NULL	Lund 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Chromosomal research in Lund gives new methods for diagnosis and therapy in cancer ) .
	manualset3
143184	3	409001	5	NULL	NULL	0	NULL	new methods 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Chromosomal research in Lund gives new methods for diagnosis and therapy in cancer ) .
	manualset3
143185	4	409001	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Chromosomal research in Lund gives new methods for diagnosis and therapy in cancer ) .
	manualset3
143186	5	409001	5	NULL	NULL	0	NULL	therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Chromosomal research in Lund gives new methods for diagnosis and therapy in cancer ) .
	manualset3
143187	6	409001	5	NULL	NULL	0	NULL	cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Chromosomal research in Lund gives new methods for diagnosis and therapy in cancer ) .
	manualset3
143188	1	409002	5	NULL	NULL	0	NULL	series 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of alkyl acyl carnitine esters ( alkyl 3-acyloxy-4-trimethylammonium butyrate chloride ) were synthesized as potential biocompatible cationic lipids for use in gene transfer .
	manualset3
143189	2	409002	5	NULL	NULL	0	NULL	alkyl acyl carnitine esters ( alkyl 3-acyloxy-4-trimethylammonium butyrate chloride )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of alkyl acyl carnitine esters ( alkyl 3-acyloxy-4-trimethylammonium butyrate chloride ) were synthesized as potential biocompatible cationic lipids for use in gene transfer .
	manualset3
143190	3	409002	5	NULL	NULL	0	NULL	potential biocompatible cationic lipids	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of alkyl acyl carnitine esters ( alkyl 3-acyloxy-4-trimethylammonium butyrate chloride ) were synthesized as potential biocompatible cationic lipids for use in gene transfer .
	manualset3
143191	4	409002	5	NULL	NULL	0	NULL	gene transfer	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of alkyl acyl carnitine esters ( alkyl 3-acyloxy-4-trimethylammonium butyrate chloride ) were synthesized as potential biocompatible cationic lipids for use in gene transfer .
	manualset3
143192	1	409003	5	NULL	NULL	0	NULL	biochemical changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The biochemical changes observed in neuronal tissues show the involvement of NO in the AlCl3 toxicity and cholinergic neurotransmission , and that L-NAME may have potential neuroprotective effects .
	manualset3
143193	2	409003	5	NULL	NULL	0	NULL	neuronal tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The biochemical changes observed in neuronal tissues show the involvement of NO in the AlCl3 toxicity and cholinergic neurotransmission , and that L-NAME may have potential neuroprotective effects .
	manualset3
143194	3	409003	5	NULL	NULL	0	NULL	involvement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The biochemical changes observed in neuronal tissues show the involvement of NO in the AlCl3 toxicity and cholinergic neurotransmission , and that L-NAME may have potential neuroprotective effects .
	manualset3
143195	4	409003	5	NULL	NULL	0	NULL	NO 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The biochemical changes observed in neuronal tissues show the involvement of NO in the AlCl3 toxicity and cholinergic neurotransmission , and that L-NAME may have potential neuroprotective effects .
	manualset3
143196	5	409003	5	NULL	NULL	0	NULL	AlCl3 toxicity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The biochemical changes observed in neuronal tissues show the involvement of NO in the AlCl3 toxicity and cholinergic neurotransmission , and that L-NAME may have potential neuroprotective effects .
	manualset3
143197	6	409003	5	NULL	NULL	0	NULL	cholinergic neurotransmission	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The biochemical changes observed in neuronal tissues show the involvement of NO in the AlCl3 toxicity and cholinergic neurotransmission , and that L-NAME may have potential neuroprotective effects .
	manualset3
143198	7	409003	5	NULL	NULL	0	NULL	L-NAME 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The biochemical changes observed in neuronal tissues show the involvement of NO in the AlCl3 toxicity and cholinergic neurotransmission , and that L-NAME may have potential neuroprotective effects .
	manualset3
143199	8	409003	5	NULL	NULL	0	NULL	potential neuroprotective effects 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The biochemical changes observed in neuronal tissues show the involvement of NO in the AlCl3 toxicity and cholinergic neurotransmission , and that L-NAME may have potential neuroprotective effects .
	manualset3
143200	1	409004	5	NULL	NULL	0	NULL	biochemistry 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The biochemistry of glucose-6-phosphate dehydrogenase , 6-phosphogluconate dehydrogenase and glutathione reductase .
	manualset3
143201	2	409004	5	NULL	NULL	0	NULL	glucose-6-phosphate dehydrogenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The biochemistry of glucose-6-phosphate dehydrogenase , 6-phosphogluconate dehydrogenase and glutathione reductase .
	manualset3
143202	3	409004	5	NULL	NULL	0	NULL	6-phosphogluconate dehydrogenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The biochemistry of glucose-6-phosphate dehydrogenase , 6-phosphogluconate dehydrogenase and glutathione reductase .
	manualset3
143203	4	409004	5	NULL	NULL	0	NULL	glutathione reductase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The biochemistry of glucose-6-phosphate dehydrogenase , 6-phosphogluconate dehydrogenase and glutathione reductase .
	manualset3
143204	1	409005	5	NULL	NULL	0	NULL	biodiversity	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The biodiversity of field margins was relatively high .
	manualset3
143205	2	409005	5	NULL	NULL	0	NULL	field margins	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The biodiversity of field margins was relatively high .
	manualset3
143206	1	409006	5	NULL	NULL	NULL	NULL	biological activity results	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The biological activity results showed that the complex at the dose of 0.25-0 .75 mg Cr/kg body weight could decrease the blood glucose level and increase liver glycogen level in alloxan-diabetic rats .
	manualset3
143207	2	409006	5	NULL	NULL	0	NULL	complex 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The biological activity results showed that the complex at the dose of 0.25-0 .75 mg Cr/kg body weight could decrease the blood glucose level and increase liver glycogen level in alloxan-diabetic rats .
	manualset3
143208	3	409006	5	NULL	NULL	0	NULL	dose 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The biological activity results showed that the complex at the dose of 0.25-0 .75 mg Cr/kg body weight could decrease the blood glucose level and increase liver glycogen level in alloxan-diabetic rats .
	manualset3
143209	4	409006	5	NULL	NULL	0	NULL	0.25-0 .75 mg Cr/kg body weight	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The biological activity results showed that the complex at the dose of 0.25-0 .75 mg Cr/kg body weight could decrease the blood glucose level and increase liver glycogen level in alloxan-diabetic rats .
	manualset3
143211	5	409006	5	NULL	NULL	NULL	NULL	blood glucose level	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The biological activity results showed that the complex at the dose of 0.25-0 .75 mg Cr/kg body weight could decrease the blood glucose level and increase liver glycogen level in alloxan-diabetic rats .
	manualset3
143212	6	409006	5	NULL	NULL	0	NULL	liver glycogen level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The biological activity results showed that the complex at the dose of 0.25-0 .75 mg Cr/kg body weight could decrease the blood glucose level and increase liver glycogen level in alloxan-diabetic rats .
	manualset3
143213	7	409006	5	NULL	NULL	0	NULL	alloxan-diabetic rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The biological activity results showed that the complex at the dose of 0.25-0 .75 mg Cr/kg body weight could decrease the blood glucose level and increase liver glycogen level in alloxan-diabetic rats .
	manualset3
143214	1	409007	5	NULL	NULL	0	NULL	biological availability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The biological availability of iron in the rhizosphere was assessed by evaluating ice nucleation activity ( INA ) expressed in situ by Pseudomonas fluorescens Pf-5 containing a transcriptional fusion ( pvd-inaZ ) of an iron-regulated promoter to an ice nucleation reporter gene ( inaZ ) .
	manualset3
143215	2	409007	5	NULL	NULL	0	NULL	iron 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The biological availability of iron in the rhizosphere was assessed by evaluating ice nucleation activity ( INA ) expressed in situ by Pseudomonas fluorescens Pf-5 containing a transcriptional fusion ( pvd-inaZ ) of an iron-regulated promoter to an ice nucleation reporter gene ( inaZ ) .
	manualset3
143216	3	409007	5	NULL	NULL	NULL	NULL	rhizosphere 	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The biological availability of iron in the rhizosphere was assessed by evaluating ice nucleation activity ( INA ) expressed in situ by Pseudomonas fluorescens Pf-5 containing a transcriptional fusion ( pvd-inaZ ) of an iron-regulated promoter to an ice nucleation reporter gene ( inaZ ) .
	manualset3
143217	4	409007	5	NULL	NULL	0	NULL	ice nucleation activity ( INA )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The biological availability of iron in the rhizosphere was assessed by evaluating ice nucleation activity ( INA ) expressed in situ by Pseudomonas fluorescens Pf-5 containing a transcriptional fusion ( pvd-inaZ ) of an iron-regulated promoter to an ice nucleation reporter gene ( inaZ ) .
	manualset3
143218	5	409007	5	NULL	NULL	0	NULL	Pseudomonas fluorescens Pf-5	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The biological availability of iron in the rhizosphere was assessed by evaluating ice nucleation activity ( INA ) expressed in situ by Pseudomonas fluorescens Pf-5 containing a transcriptional fusion ( pvd-inaZ ) of an iron-regulated promoter to an ice nucleation reporter gene ( inaZ ) .
	manualset3
143219	6	409007	5	NULL	NULL	0	NULL	transcriptional fusion ( pvd-inaZ )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The biological availability of iron in the rhizosphere was assessed by evaluating ice nucleation activity ( INA ) expressed in situ by Pseudomonas fluorescens Pf-5 containing a transcriptional fusion ( pvd-inaZ ) of an iron-regulated promoter to an ice nucleation reporter gene ( inaZ ) .
	manualset3
143220	7	409007	5	NULL	NULL	0	NULL	iron-regulated promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The biological availability of iron in the rhizosphere was assessed by evaluating ice nucleation activity ( INA ) expressed in situ by Pseudomonas fluorescens Pf-5 containing a transcriptional fusion ( pvd-inaZ ) of an iron-regulated promoter to an ice nucleation reporter gene ( inaZ ) .
	manualset3
143221	8	409007	5	NULL	NULL	0	NULL	ice nucleation reporter gene ( inaZ )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The biological availability of iron in the rhizosphere was assessed by evaluating ice nucleation activity ( INA ) expressed in situ by Pseudomonas fluorescens Pf-5 containing a transcriptional fusion ( pvd-inaZ ) of an iron-regulated promoter to an ice nucleation reporter gene ( inaZ ) .
	manualset3
143222	1	409008	5	NULL	NULL	0	NULL	biological half-life 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The biological half-life and the final residue level were investigated using Aster scaber over a 10-days cultivation period .
	manualset3
143223	2	409008	5	NULL	NULL	0	NULL	final residue level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The biological half-life and the final residue level were investigated using Aster scaber over a 10-days cultivation period .
	manualset3
143224	3	409008	5	NULL	NULL	0	NULL	Aster scaber	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The biological half-life and the final residue level were investigated using Aster scaber over a 10-days cultivation period .
	manualset3
143225	4	409008	5	NULL	NULL	0	NULL	10-days cultivation period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The biological half-life and the final residue level were investigated using Aster scaber over a 10-days cultivation period .
	manualset3
143226	1	409009	5	NULL	NULL	0	NULL	biological properties 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The biological properties of human T-cell leukemia virus type I ( HTLV-I ) and HTLV type II ( HTLV-II ) are not well elucidated as cell-free viruses .
	manualset3
143227	2	409009	5	NULL	NULL	0	NULL	human T-cell leukemia virus type I ( HTLV-I )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The biological properties of human T-cell leukemia virus type I ( HTLV-I ) and HTLV type II ( HTLV-II ) are not well elucidated as cell-free viruses .
	manualset3
143228	3	409009	5	NULL	NULL	0	NULL	HTLV type II ( HTLV-II )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The biological properties of human T-cell leukemia virus type I ( HTLV-I ) and HTLV type II ( HTLV-II ) are not well elucidated as cell-free viruses .
	manualset3
143229	4	409009	5	NULL	NULL	0	NULL	cell-free viruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The biological properties of human T-cell leukemia virus type I ( HTLV-I ) and HTLV type II ( HTLV-II ) are not well elucidated as cell-free viruses .
	manualset3
143230	1	409010	5	NULL	NULL	0	NULL	biological roles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The biological roles of Ikaros include regulating the development and function of the immune system and acting as a master regulator of hematopoietic differentiation .
	manualset3
143231	2	409010	5	NULL	NULL	NULL	NULL	Ikaros 	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The biological roles of Ikaros include regulating the development and function of the immune system and acting as a master regulator of hematopoietic differentiation .
	manualset3
143232	3	409010	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The biological roles of Ikaros include regulating the development and function of the immune system and acting as a master regulator of hematopoietic differentiation .
	manualset3
143233	4	409010	5	NULL	NULL	0	NULL	function 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The biological roles of Ikaros include regulating the development and function of the immune system and acting as a master regulator of hematopoietic differentiation .
	manualset3
143234	5	409010	5	NULL	NULL	0	NULL	immune system	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The biological roles of Ikaros include regulating the development and function of the immune system and acting as a master regulator of hematopoietic differentiation .
	manualset3
143235	6	409010	5	NULL	NULL	0	NULL	master regulator	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The biological roles of Ikaros include regulating the development and function of the immune system and acting as a master regulator of hematopoietic differentiation .
	manualset3
143236	7	409010	5	NULL	NULL	0	NULL	hematopoietic differentiation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The biological roles of Ikaros include regulating the development and function of the immune system and acting as a master regulator of hematopoietic differentiation .
	manualset3
143237	1	409011	5	NULL	NULL	0	NULL	biomedical model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The biomedical model has successfully reduced mother and child mortality and diseases during the labor and puerperal period .
	manualset3
143238	2	409011	5	NULL	NULL	0	NULL	mother mortality 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The biomedical model has successfully reduced mother and child mortality and diseases during the labor and puerperal period .
	manualset3
143239	3	409011	5	NULL	NULL	0	NULL	child mortality 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The biomedical model has successfully reduced mother and child mortality and diseases during the labor and puerperal period .
	manualset3
143240	4	409011	5	NULL	NULL	0	NULL	diseases 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The biomedical model has successfully reduced mother and child mortality and diseases during the labor and puerperal period .
	manualset3
143241	5	409011	5	NULL	NULL	0	NULL	labor 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The biomedical model has successfully reduced mother and child mortality and diseases during the labor and puerperal period .
	manualset3
143242	6	409011	5	NULL	NULL	0	NULL	puerperal period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The biomedical model has successfully reduced mother and child mortality and diseases during the labor and puerperal period .
	manualset3
143243	1	409012	5	NULL	NULL	0	NULL	birth season 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The birth season starts in December and ends in June , with a peak from March to May , and a median birth date of April 10 .
	manualset3
143244	2	409012	5	NULL	NULL	0	NULL	December 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	The birth season starts in December and ends in June , with a peak from March to May , and a median birth date of April 10 .
	manualset3
143245	3	409012	5	NULL	NULL	0	NULL	June 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	The birth season starts in December and ends in June , with a peak from March to May , and a median birth date of April 10 .
	manualset3
143246	4	409012	5	NULL	NULL	0	NULL	March 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	The birth season starts in December and ends in June , with a peak from March to May , and a median birth date of April 10 .
	manualset3
143247	5	409012	5	NULL	NULL	0	NULL	May 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	The birth season starts in December and ends in June , with a peak from March to May , and a median birth date of April 10 .
	manualset3
143248	6	409012	5	NULL	NULL	0	NULL	median birth date	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	The birth season starts in December and ends in June , with a peak from March to May , and a median birth date of April 10 .
	manualset3
143249	7	409012	5	NULL	NULL	0	NULL	April 10	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	The birth season starts in December and ends in June , with a peak from March to May , and a median birth date of April 10 .
	manualset3
143250	1	409013	5	NULL	NULL	0	NULL	 bis-acylureas	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The bis-acylureas have two acylurea groups , - NH-CO-NH-CO - , divided by a pentamethylene spacer , - ( CH ( 2 ) ) ( 5 ) - , and two symmetric functional end groups , such as , aliphatic , benzyl , mono - and bi-thiophenyl , sulfur-containing , and propargyl ( HC ( triple bond ) CCH ( 2 ) - ) moieties .
	manualset3
143251	2	409013	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The bis-acylureas have two acylurea groups , - NH-CO-NH-CO - , divided by a pentamethylene spacer , - ( CH ( 2 ) ) ( 5 ) - , and two symmetric functional end groups , such as , aliphatic , benzyl , mono - and bi-thiophenyl , sulfur-containing , and propargyl ( HC ( triple bond ) CCH ( 2 ) - ) moieties .
	manualset3
143252	3	409013	5	NULL	NULL	0	NULL	acylurea groups , - NH-CO-NH-CO - 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The bis-acylureas have two acylurea groups , - NH-CO-NH-CO - , divided by a pentamethylene spacer , - ( CH ( 2 ) ) ( 5 ) - , and two symmetric functional end groups , such as , aliphatic , benzyl , mono - and bi-thiophenyl , sulfur-containing , and propargyl ( HC ( triple bond ) CCH ( 2 ) - ) moieties .
	manualset3
143253	4	409013	5	NULL	NULL	0	NULL	pentamethylene spacer , - ( CH ( 2 ) ) ( 5 ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The bis-acylureas have two acylurea groups , - NH-CO-NH-CO - , divided by a pentamethylene spacer , - ( CH ( 2 ) ) ( 5 ) - , and two symmetric functional end groups , such as , aliphatic , benzyl , mono - and bi-thiophenyl , sulfur-containing , and propargyl ( HC ( triple bond ) CCH ( 2 ) - ) moieties .
	manualset3
143254	5	409013	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The bis-acylureas have two acylurea groups , - NH-CO-NH-CO - , divided by a pentamethylene spacer , - ( CH ( 2 ) ) ( 5 ) - , and two symmetric functional end groups , such as , aliphatic , benzyl , mono - and bi-thiophenyl , sulfur-containing , and propargyl ( HC ( triple bond ) CCH ( 2 ) - ) moieties .
	manualset3
143255	6	409013	5	NULL	NULL	0	NULL	symmetric functional end groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The bis-acylureas have two acylurea groups , - NH-CO-NH-CO - , divided by a pentamethylene spacer , - ( CH ( 2 ) ) ( 5 ) - , and two symmetric functional end groups , such as , aliphatic , benzyl , mono - and bi-thiophenyl , sulfur-containing , and propargyl ( HC ( triple bond ) CCH ( 2 ) - ) moieties .
	manualset3
143256	7	409013	5	NULL	NULL	0	NULL	aliphatic moieties 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The bis-acylureas have two acylurea groups , - NH-CO-NH-CO - , divided by a pentamethylene spacer , - ( CH ( 2 ) ) ( 5 ) - , and two symmetric functional end groups , such as , aliphatic , benzyl , mono - and bi-thiophenyl , sulfur-containing , and propargyl ( HC ( triple bond ) CCH ( 2 ) - ) moieties .
	manualset3
143257	8	409013	5	NULL	NULL	0	NULL	benzyl moieties 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The bis-acylureas have two acylurea groups , - NH-CO-NH-CO - , divided by a pentamethylene spacer , - ( CH ( 2 ) ) ( 5 ) - , and two symmetric functional end groups , such as , aliphatic , benzyl , mono - and bi-thiophenyl , sulfur-containing , and propargyl ( HC ( triple bond ) CCH ( 2 ) - ) moieties .
	manualset3
143258	9	409013	5	NULL	NULL	0	NULL	mono - thiophenyl moieties 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The bis-acylureas have two acylurea groups , - NH-CO-NH-CO - , divided by a pentamethylene spacer , - ( CH ( 2 ) ) ( 5 ) - , and two symmetric functional end groups , such as , aliphatic , benzyl , mono - and bi-thiophenyl , sulfur-containing , and propargyl ( HC ( triple bond ) CCH ( 2 ) - ) moieties .
	manualset3
143259	10	409013	5	NULL	NULL	0	NULL	 bi-thiophenyl moieties 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The bis-acylureas have two acylurea groups , - NH-CO-NH-CO - , divided by a pentamethylene spacer , - ( CH ( 2 ) ) ( 5 ) - , and two symmetric functional end groups , such as , aliphatic , benzyl , mono - and bi-thiophenyl , sulfur-containing , and propargyl ( HC ( triple bond ) CCH ( 2 ) - ) moieties .
	manualset3
143260	11	409013	5	NULL	NULL	0	NULL	sulfur-containing moieties 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The bis-acylureas have two acylurea groups , - NH-CO-NH-CO - , divided by a pentamethylene spacer , - ( CH ( 2 ) ) ( 5 ) - , and two symmetric functional end groups , such as , aliphatic , benzyl , mono - and bi-thiophenyl , sulfur-containing , and propargyl ( HC ( triple bond ) CCH ( 2 ) - ) moieties .
	manualset3
143261	12	409013	5	NULL	NULL	0	NULL	propargyl ( HC ( triple bond ) CCH ( 2 ) - ) moieties	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The bis-acylureas have two acylurea groups , - NH-CO-NH-CO - , divided by a pentamethylene spacer , - ( CH ( 2 ) ) ( 5 ) - , and two symmetric functional end groups , such as , aliphatic , benzyl , mono - and bi-thiophenyl , sulfur-containing , and propargyl ( HC ( triple bond ) CCH ( 2 ) - ) moieties .
	manualset3
143262	1	409014	5	NULL	NULL	0	NULL	bis ( 2-ethylhexyl ) phthalate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The bis ( 2-ethylhexyl ) phthalate was solubilized with polysorbate 80 .
	manualset3
143263	2	409014	5	NULL	NULL	0	NULL	polysorbate 80	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The bis ( 2-ethylhexyl ) phthalate was solubilized with polysorbate 80 .
	manualset3
143264	1	409015	5	NULL	NULL	0	NULL	 blood-nerve barrier	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The blood-nerve barrier of nerve allografts at 2 and 6 weeks postoperatively was permeable to intravenously injected horseradish peroxidase , which spread into endoneurial tissue .
	manualset3
143265	2	409015	5	NULL	NULL	0	NULL	nerve allografts	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The blood-nerve barrier of nerve allografts at 2 and 6 weeks postoperatively was permeable to intravenously injected horseradish peroxidase , which spread into endoneurial tissue .
	manualset3
143266	3	409015	5	NULL	NULL	0	NULL	2 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The blood-nerve barrier of nerve allografts at 2 and 6 weeks postoperatively was permeable to intravenously injected horseradish peroxidase , which spread into endoneurial tissue .
	manualset3
143267	4	409015	5	NULL	NULL	0	NULL	6 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The blood-nerve barrier of nerve allografts at 2 and 6 weeks postoperatively was permeable to intravenously injected horseradish peroxidase , which spread into endoneurial tissue .
	manualset3
143268	5	409015	5	NULL	NULL	0	NULL	intravenously injected horseradish peroxidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The blood-nerve barrier of nerve allografts at 2 and 6 weeks postoperatively was permeable to intravenously injected horseradish peroxidase , which spread into endoneurial tissue .
	manualset3
143269	6	409015	5	NULL	NULL	0	NULL	endoneurial tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The blood-nerve barrier of nerve allografts at 2 and 6 weeks postoperatively was permeable to intravenously injected horseradish peroxidase , which spread into endoneurial tissue .
	manualset3
143270	1	409016	5	NULL	NULL	0	NULL	blood amino acid concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The blood amino acid concentration in diabetic patients is , however , reduced , which suggests that the hepatic uptake of amino acids is accelerated .
	manualset3
143271	2	409016	5	NULL	NULL	0	NULL	diabetic patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The blood amino acid concentration in diabetic patients is , however , reduced , which suggests that the hepatic uptake of amino acids is accelerated .
	manualset3
143272	3	409016	5	NULL	NULL	NULL	NULL	hepatic uptake	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The blood amino acid concentration in diabetic patients is , however , reduced , which suggests that the hepatic uptake of amino acids is accelerated .
	manualset3
143273	4	409016	5	NULL	NULL	0	NULL	amino acids 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The blood amino acid concentration in diabetic patients is , however , reduced , which suggests that the hepatic uptake of amino acids is accelerated .
	manualset3
143274	1	409017	5	NULL	NULL	0	NULL	blood ethanol concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The blood and urine ethanol concentrations were low 0.096 and 0.100 g/L , respectively .
	manualset3
143275	2	409017	5	NULL	NULL	0	NULL	urine ethanol concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The blood and urine ethanol concentrations were low 0.096 and 0.100 g/L , respectively .
	manualset3
143276	3	409017	5	NULL	NULL	0	NULL	0.096 g/L 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The blood and urine ethanol concentrations were low 0.096 and 0.100 g/L , respectively .
	manualset3
143277	4	409017	5	NULL	NULL	0	NULL	0.100 g/L 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The blood and urine ethanol concentrations were low 0.096 and 0.100 g/L , respectively .
	manualset3
143278	1	409018	5	NULL	NULL	0	NULL	series 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of experiments to explore the cellular basis of the carotenoid accumulation induced by the Or gene was completed .
	manualset3
143279	2	409018	5	NULL	NULL	0	NULL	experiments 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of experiments to explore the cellular basis of the carotenoid accumulation induced by the Or gene was completed .
	manualset3
143280	3	409018	5	NULL	NULL	0	NULL	cellular basis	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of experiments to explore the cellular basis of the carotenoid accumulation induced by the Or gene was completed .
	manualset3
143281	4	409018	5	NULL	NULL	0	NULL	carotenoid accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of experiments to explore the cellular basis of the carotenoid accumulation induced by the Or gene was completed .
	manualset3
143282	5	409018	5	NULL	NULL	0	NULL	Or gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of experiments to explore the cellular basis of the carotenoid accumulation induced by the Or gene was completed .
	manualset3
143283	1	409019	5	NULL	NULL	0	NULL	blood glucose monitoring devices ( BGMDs ) 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The blood glucose monitoring devices ( BGMDs ) are an integral part of diabetes management now-a-days .
	manualset3
143284	2	409019	5	NULL	NULL	0	NULL	diabetes management 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The blood glucose monitoring devices ( BGMDs ) are an integral part of diabetes management now-a-days .
	manualset3
143285	1	409020	5	NULL	NULL	0	NULL	blood glucose response 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The blood glucose response to a brief infusion of insulin ( 0.012 U/kg body wt ) was studied in the initial phase of Type 1 diabetes in 21 children and in 20 healthy controls .
	manualset3
143286	2	409020	5	NULL	NULL	0	NULL	infusion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The blood glucose response to a brief infusion of insulin ( 0.012 U/kg body wt ) was studied in the initial phase of Type 1 diabetes in 21 children and in 20 healthy controls .
	manualset3
143287	3	409020	5	NULL	NULL	0	NULL	insulin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The blood glucose response to a brief infusion of insulin ( 0.012 U/kg body wt ) was studied in the initial phase of Type 1 diabetes in 21 children and in 20 healthy controls .
	manualset3
143288	4	409020	5	NULL	NULL	0	NULL	0.012 U/kg body wt	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The blood glucose response to a brief infusion of insulin ( 0.012 U/kg body wt ) was studied in the initial phase of Type 1 diabetes in 21 children and in 20 healthy controls .
	manualset3
143289	5	409020	5	NULL	NULL	0	NULL	initial phase	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The blood glucose response to a brief infusion of insulin ( 0.012 U/kg body wt ) was studied in the initial phase of Type 1 diabetes in 21 children and in 20 healthy controls .
	manualset3
143290	6	409020	5	NULL	NULL	0	NULL	Type 1 diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The blood glucose response to a brief infusion of insulin ( 0.012 U/kg body wt ) was studied in the initial phase of Type 1 diabetes in 21 children and in 20 healthy controls .
	manualset3
143291	7	409020	5	NULL	NULL	0	NULL	21 children	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The blood glucose response to a brief infusion of insulin ( 0.012 U/kg body wt ) was studied in the initial phase of Type 1 diabetes in 21 children and in 20 healthy controls .
	manualset3
143292	8	409020	5	NULL	NULL	0	NULL	20 healthy controls	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The blood glucose response to a brief infusion of insulin ( 0.012 U/kg body wt ) was studied in the initial phase of Type 1 diabetes in 21 children and in 20 healthy controls .
	manualset3
143293	1	409021	5	NULL	NULL	0	NULL	blue-light photoreceptor , cryptochrome ( CRY ) 2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The blue-light photoreceptors , cryptochrome ( CRY ) 2 and phototropin ( PHOT ) 2 , are specifically required for maintaining the stability of the R protein HRT , and thereby resistance to TCV .
	manualset3
143294	2	409021	5	NULL	NULL	0	NULL	blue-light photoreceptor, phototropin ( PHOT ) 2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The blue-light photoreceptors , cryptochrome ( CRY ) 2 and phototropin ( PHOT ) 2 , are specifically required for maintaining the stability of the R protein HRT , and thereby resistance to TCV .
	manualset3
143295	3	409021	5	NULL	NULL	0	NULL	stability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The blue-light photoreceptors , cryptochrome ( CRY ) 2 and phototropin ( PHOT ) 2 , are specifically required for maintaining the stability of the R protein HRT , and thereby resistance to TCV .
	manualset3
143296	4	409021	5	NULL	NULL	0	NULL	R protein HRT 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The blue-light photoreceptors , cryptochrome ( CRY ) 2 and phototropin ( PHOT ) 2 , are specifically required for maintaining the stability of the R protein HRT , and thereby resistance to TCV .
	manualset3
143297	5	409021	5	NULL	NULL	0	NULL	resistance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The blue-light photoreceptors , cryptochrome ( CRY ) 2 and phototropin ( PHOT ) 2 , are specifically required for maintaining the stability of the R protein HRT , and thereby resistance to TCV .
	manualset3
143298	6	409021	5	NULL	NULL	0	NULL	TCV 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The blue-light photoreceptors , cryptochrome ( CRY ) 2 and phototropin ( PHOT ) 2 , are specifically required for maintaining the stability of the R protein HRT , and thereby resistance to TCV .
	manualset3
143299	1	409022	5	NULL	NULL	0	NULL	bone defect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The bone defect was substituted with hydroxylapatit ceramic .
	manualset3
143300	2	409022	5	NULL	NULL	0	NULL	hydroxylapatit ceramic	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The bone defect was substituted with hydroxylapatit ceramic .
	manualset3
143301	1	409023	5	NULL	NULL	0	NULL	borer 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The borer was distributed across the whole country , and at maturity an average 25 % of the ears sampled in maize fields were infested .
	manualset3
143302	2	409023	5	NULL	NULL	0	NULL	country 	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The borer was distributed across the whole country , and at maturity an average 25 % of the ears sampled in maize fields were infested .
	manualset3
143303	3	409023	5	NULL	NULL	0	NULL	maturity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The borer was distributed across the whole country , and at maturity an average 25 % of the ears sampled in maize fields were infested .
	manualset3
143304	4	409023	5	NULL	NULL	0	NULL	average 25 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The borer was distributed across the whole country , and at maturity an average 25 % of the ears sampled in maize fields were infested .
	manualset3
143305	5	409023	5	NULL	NULL	0	NULL	ears 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The borer was distributed across the whole country , and at maturity an average 25 % of the ears sampled in maize fields were infested .
	manualset3
143306	6	409023	5	NULL	NULL	0	NULL	maize fields 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The borer was distributed across the whole country , and at maturity an average 25 % of the ears sampled in maize fields were infested .
	manualset3
143307	1	409024	5	NULL	NULL	0	NULL	bound lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The bound lymphocytes released by human or dog IgG recovered 60-70 % of the B-cells without significantly impairing the cell viability .
	manualset3
143308	2	409024	5	NULL	NULL	0	NULL	human IgG 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The bound lymphocytes released by human or dog IgG recovered 60-70 % of the B-cells without significantly impairing the cell viability .
	manualset3
143309	3	409024	5	NULL	NULL	0	NULL	dog IgG 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The bound lymphocytes released by human or dog IgG recovered 60-70 % of the B-cells without significantly impairing the cell viability .
	manualset3
143310	4	409024	5	NULL	NULL	0	NULL	60-70 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The bound lymphocytes released by human or dog IgG recovered 60-70 % of the B-cells without significantly impairing the cell viability .
	manualset3
143311	5	409024	5	NULL	NULL	0	NULL	B-cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The bound lymphocytes released by human or dog IgG recovered 60-70 % of the B-cells without significantly impairing the cell viability .
	manualset3
143312	6	409024	5	NULL	NULL	0	NULL	cell viability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The bound lymphocytes released by human or dog IgG recovered 60-70 % of the B-cells without significantly impairing the cell viability .
	manualset3
143313	1	409025	5	NULL	NULL	0	NULL	boundaries 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The boundaries between the person and the world .
	manualset3
143314	2	409025	5	NULL	NULL	0	NULL	person 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The boundaries between the person and the world .
	manualset3
143315	3	409025	5	NULL	NULL	0	NULL	world 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The boundaries between the person and the world .
	manualset3
143316	1	409026	5	NULL	NULL	0	NULL	boy 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The boy died after 38 days because of a hemorrhage of the lungs .
	manualset3
143317	2	409026	5	NULL	NULL	0	NULL	38 days 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The boy died after 38 days because of a hemorrhage of the lungs .
	manualset3
143318	3	409026	5	NULL	NULL	0	NULL	hemorrhage 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The boy died after 38 days because of a hemorrhage of the lungs .
	manualset3
143319	4	409026	5	NULL	NULL	0	NULL	lungs 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The boy died after 38 days because of a hemorrhage of the lungs .
	manualset3
143320	1	409027	5	NULL	NULL	0	NULL	brain NO system	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The brain NO system is affected by several currently used cardiovascular drugs and accordingly it has been suggested that central action of NO may contribute to their therapeutics effects .
	manualset3
143321	2	409027	5	NULL	NULL	0	NULL	cardiovascular drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The brain NO system is affected by several currently used cardiovascular drugs and accordingly it has been suggested that central action of NO may contribute to their therapeutics effects .
	manualset3
143322	3	409027	5	NULL	NULL	0	NULL	central action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The brain NO system is affected by several currently used cardiovascular drugs and accordingly it has been suggested that central action of NO may contribute to their therapeutics effects .
	manualset3
143323	4	409027	5	NULL	NULL	0	NULL	NO 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The brain NO system is affected by several currently used cardiovascular drugs and accordingly it has been suggested that central action of NO may contribute to their therapeutics effects .
	manualset3
143324	5	409027	5	NULL	NULL	0	NULL	therapeutics effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The brain NO system is affected by several currently used cardiovascular drugs and accordingly it has been suggested that central action of NO may contribute to their therapeutics effects .
	manualset3
143325	1	409028	5	NULL	NULL	0	NULL	breakdown 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The breakdown of lignin by fungi is a key step during carbon recycling in terrestrial ecosystems .
	manualset3
143326	2	409028	5	NULL	NULL	0	NULL	lignin 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The breakdown of lignin by fungi is a key step during carbon recycling in terrestrial ecosystems .
	manualset3
143327	3	409028	5	NULL	NULL	0	NULL	fungi 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The breakdown of lignin by fungi is a key step during carbon recycling in terrestrial ecosystems .
	manualset3
143328	4	409028	5	NULL	NULL	0	NULL	key step 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The breakdown of lignin by fungi is a key step during carbon recycling in terrestrial ecosystems .
	manualset3
143329	5	409028	5	NULL	NULL	0	NULL	carbon recycling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The breakdown of lignin by fungi is a key step during carbon recycling in terrestrial ecosystems .
	manualset3
143330	6	409028	5	NULL	NULL	0	NULL	terrestrial ecosystems	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The breakdown of lignin by fungi is a key step during carbon recycling in terrestrial ecosystems .
	manualset3
143331	1	409029	5	NULL	NULL	0	NULL	brominated coumarins	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The brominated coumarins can be diversified by reduction of the Pd ( II ) catalyst to Pd ( 0 ) followed by Suzuki , Sonogashira , Heck , or Hartwig-Buchwald coupling .
	manualset3
143332	2	409029	5	NULL	NULL	0	NULL	reduction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The brominated coumarins can be diversified by reduction of the Pd ( II ) catalyst to Pd ( 0 ) followed by Suzuki , Sonogashira , Heck , or Hartwig-Buchwald coupling .
	manualset3
143333	3	409029	5	NULL	NULL	0	NULL	Pd ( II ) catalyst	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The brominated coumarins can be diversified by reduction of the Pd ( II ) catalyst to Pd ( 0 ) followed by Suzuki , Sonogashira , Heck , or Hartwig-Buchwald coupling .
	manualset3
143334	4	409029	5	NULL	NULL	0	NULL	Pd ( 0 )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The brominated coumarins can be diversified by reduction of the Pd ( II ) catalyst to Pd ( 0 ) followed by Suzuki , Sonogashira , Heck , or Hartwig-Buchwald coupling .
	manualset3
143335	5	409029	5	NULL	NULL	0	NULL	Suzuki coupling 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The brominated coumarins can be diversified by reduction of the Pd ( II ) catalyst to Pd ( 0 ) followed by Suzuki , Sonogashira , Heck , or Hartwig-Buchwald coupling .
	manualset3
143336	6	409029	5	NULL	NULL	0	NULL	Sonogashira coupling 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The brominated coumarins can be diversified by reduction of the Pd ( II ) catalyst to Pd ( 0 ) followed by Suzuki , Sonogashira , Heck , or Hartwig-Buchwald coupling .
	manualset3
143337	7	409029	5	NULL	NULL	0	NULL	Heck coupling 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The brominated coumarins can be diversified by reduction of the Pd ( II ) catalyst to Pd ( 0 ) followed by Suzuki , Sonogashira , Heck , or Hartwig-Buchwald coupling .
	manualset3
143338	8	409029	5	NULL	NULL	0	NULL	Hartwig-Buchwald coupling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The brominated coumarins can be diversified by reduction of the Pd ( II ) catalyst to Pd ( 0 ) followed by Suzuki , Sonogashira , Heck , or Hartwig-Buchwald coupling .
	manualset3
143339	1	409030	5	NULL	NULL	0	NULL	broth macrodilution reference method 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The broth macrodilution reference method of the National Committee for Clinical Laboratory Standards ( NCCLS , M27-P ) was adapted to the microdilution method .
	manualset3
143340	2	409030	5	NULL	NULL	0	NULL	National Committee for Clinical Laboratory Standards ( NCCLS , M27-P ) 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The broth macrodilution reference method of the National Committee for Clinical Laboratory Standards ( NCCLS , M27-P ) was adapted to the microdilution method .
	manualset3
143341	3	409030	5	NULL	NULL	0	NULL	microdilution method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The broth macrodilution reference method of the National Committee for Clinical Laboratory Standards ( NCCLS , M27-P ) was adapted to the microdilution method .
	manualset3
143342	1	409031	5	NULL	NULL	0	NULL	buffering 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The buffering and excretion of acids .
	manualset3
143343	2	409031	5	NULL	NULL	0	NULL	excretion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The buffering and excretion of acids .
	manualset3
143344	3	409031	5	NULL	NULL	0	NULL	acids 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The buffering and excretion of acids .
	manualset3
143345	1	409032	5	NULL	NULL	0	NULL	( 1-24 ) corticotrophin-tetracosapeptide ( batch 000179 )	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The bulk ( 1-24 ) corticotrophin-tetracosapeptide ( batch 000179 ) from which the IRP was prepared contained 10.4 % ( w/w ) acetic acid and 8.3 % ( w/w ) water ; its ( 1-24 ) corticotrophin-tetracosapeptide content was estimated to be 71.7 % ( w/w ) by amino acid analysis , 74.2 % ( w/w ) by high performance liquid chromatography ( HPLC ) and 77.5 % ( w/w ) by spectrophotometry .
	manualset3
143346	2	409032	5	NULL	NULL	0	NULL	IRP 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The bulk ( 1-24 ) corticotrophin-tetracosapeptide ( batch 000179 ) from which the IRP was prepared contained 10.4 % ( w/w ) acetic acid and 8.3 % ( w/w ) water ; its ( 1-24 ) corticotrophin-tetracosapeptide content was estimated to be 71.7 % ( w/w ) by amino acid analysis , 74.2 % ( w/w ) by high performance liquid chromatography ( HPLC ) and 77.5 % ( w/w ) by spectrophotometry .
	manualset3
143347	3	409032	5	NULL	NULL	0	NULL	 10.4 % ( w/w ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The bulk ( 1-24 ) corticotrophin-tetracosapeptide ( batch 000179 ) from which the IRP was prepared contained 10.4 % ( w/w ) acetic acid and 8.3 % ( w/w ) water ; its ( 1-24 ) corticotrophin-tetracosapeptide content was estimated to be 71.7 % ( w/w ) by amino acid analysis , 74.2 % ( w/w ) by high performance liquid chromatography ( HPLC ) and 77.5 % ( w/w ) by spectrophotometry .
	manualset3
143348	4	409032	5	NULL	NULL	0	NULL	acetic acid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The bulk ( 1-24 ) corticotrophin-tetracosapeptide ( batch 000179 ) from which the IRP was prepared contained 10.4 % ( w/w ) acetic acid and 8.3 % ( w/w ) water ; its ( 1-24 ) corticotrophin-tetracosapeptide content was estimated to be 71.7 % ( w/w ) by amino acid analysis , 74.2 % ( w/w ) by high performance liquid chromatography ( HPLC ) and 77.5 % ( w/w ) by spectrophotometry .
	manualset3
143349	5	409032	5	NULL	NULL	0	NULL	 8.3 % ( w/w )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The bulk ( 1-24 ) corticotrophin-tetracosapeptide ( batch 000179 ) from which the IRP was prepared contained 10.4 % ( w/w ) acetic acid and 8.3 % ( w/w ) water ; its ( 1-24 ) corticotrophin-tetracosapeptide content was estimated to be 71.7 % ( w/w ) by amino acid analysis , 74.2 % ( w/w ) by high performance liquid chromatography ( HPLC ) and 77.5 % ( w/w ) by spectrophotometry .
	manualset3
143350	6	409032	5	NULL	NULL	0	NULL	water 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The bulk ( 1-24 ) corticotrophin-tetracosapeptide ( batch 000179 ) from which the IRP was prepared contained 10.4 % ( w/w ) acetic acid and 8.3 % ( w/w ) water ; its ( 1-24 ) corticotrophin-tetracosapeptide content was estimated to be 71.7 % ( w/w ) by amino acid analysis , 74.2 % ( w/w ) by high performance liquid chromatography ( HPLC ) and 77.5 % ( w/w ) by spectrophotometry .
	manualset3
143351	7	409032	5	NULL	NULL	0	NULL	( 1-24 ) corticotrophin-tetracosapeptide content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The bulk ( 1-24 ) corticotrophin-tetracosapeptide ( batch 000179 ) from which the IRP was prepared contained 10.4 % ( w/w ) acetic acid and 8.3 % ( w/w ) water ; its ( 1-24 ) corticotrophin-tetracosapeptide content was estimated to be 71.7 % ( w/w ) by amino acid analysis , 74.2 % ( w/w ) by high performance liquid chromatography ( HPLC ) and 77.5 % ( w/w ) by spectrophotometry .
	manualset3
143352	8	409032	5	NULL	NULL	0	NULL	71.7 % ( w/w ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The bulk ( 1-24 ) corticotrophin-tetracosapeptide ( batch 000179 ) from which the IRP was prepared contained 10.4 % ( w/w ) acetic acid and 8.3 % ( w/w ) water ; its ( 1-24 ) corticotrophin-tetracosapeptide content was estimated to be 71.7 % ( w/w ) by amino acid analysis , 74.2 % ( w/w ) by high performance liquid chromatography ( HPLC ) and 77.5 % ( w/w ) by spectrophotometry .
	manualset3
143353	9	409032	5	NULL	NULL	0	NULL	amino acid analysis 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The bulk ( 1-24 ) corticotrophin-tetracosapeptide ( batch 000179 ) from which the IRP was prepared contained 10.4 % ( w/w ) acetic acid and 8.3 % ( w/w ) water ; its ( 1-24 ) corticotrophin-tetracosapeptide content was estimated to be 71.7 % ( w/w ) by amino acid analysis , 74.2 % ( w/w ) by high performance liquid chromatography ( HPLC ) and 77.5 % ( w/w ) by spectrophotometry .
	manualset3
143354	10	409032	5	NULL	NULL	0	NULL	74.2 % ( w/w )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The bulk ( 1-24 ) corticotrophin-tetracosapeptide ( batch 000179 ) from which the IRP was prepared contained 10.4 % ( w/w ) acetic acid and 8.3 % ( w/w ) water ; its ( 1-24 ) corticotrophin-tetracosapeptide content was estimated to be 71.7 % ( w/w ) by amino acid analysis , 74.2 % ( w/w ) by high performance liquid chromatography ( HPLC ) and 77.5 % ( w/w ) by spectrophotometry .
	manualset3
143355	11	409032	5	NULL	NULL	0	NULL	high performance liquid chromatography ( HPLC ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The bulk ( 1-24 ) corticotrophin-tetracosapeptide ( batch 000179 ) from which the IRP was prepared contained 10.4 % ( w/w ) acetic acid and 8.3 % ( w/w ) water ; its ( 1-24 ) corticotrophin-tetracosapeptide content was estimated to be 71.7 % ( w/w ) by amino acid analysis , 74.2 % ( w/w ) by high performance liquid chromatography ( HPLC ) and 77.5 % ( w/w ) by spectrophotometry .
	manualset3
143356	12	409032	5	NULL	NULL	0	NULL	77.5 % ( w/w ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The bulk ( 1-24 ) corticotrophin-tetracosapeptide ( batch 000179 ) from which the IRP was prepared contained 10.4 % ( w/w ) acetic acid and 8.3 % ( w/w ) water ; its ( 1-24 ) corticotrophin-tetracosapeptide content was estimated to be 71.7 % ( w/w ) by amino acid analysis , 74.2 % ( w/w ) by high performance liquid chromatography ( HPLC ) and 77.5 % ( w/w ) by spectrophotometry .
	manualset3
143357	13	409032	5	NULL	NULL	0	NULL	spectrophotometry 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The bulk ( 1-24 ) corticotrophin-tetracosapeptide ( batch 000179 ) from which the IRP was prepared contained 10.4 % ( w/w ) acetic acid and 8.3 % ( w/w ) water ; its ( 1-24 ) corticotrophin-tetracosapeptide content was estimated to be 71.7 % ( w/w ) by amino acid analysis , 74.2 % ( w/w ) by high performance liquid chromatography ( HPLC ) and 77.5 % ( w/w ) by spectrophotometry .
	manualset3
143358	1	409033	5	NULL	NULL	0	NULL	series 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of experiments was performed to determine the parameters necessary to produce immediate measurable changes in the visual system of nonhuman primates after exposure of the fovea to laser radiation .
	manualset3
143359	2	409033	5	NULL	NULL	0	NULL	experiments 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of experiments was performed to determine the parameters necessary to produce immediate measurable changes in the visual system of nonhuman primates after exposure of the fovea to laser radiation .
	manualset3
143360	3	409033	5	NULL	NULL	0	NULL	parameters 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of experiments was performed to determine the parameters necessary to produce immediate measurable changes in the visual system of nonhuman primates after exposure of the fovea to laser radiation .
	manualset3
143361	4	409033	5	NULL	NULL	0	NULL	measurable changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of experiments was performed to determine the parameters necessary to produce immediate measurable changes in the visual system of nonhuman primates after exposure of the fovea to laser radiation .
	manualset3
143362	5	409033	5	NULL	NULL	0	NULL	visual system	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of experiments was performed to determine the parameters necessary to produce immediate measurable changes in the visual system of nonhuman primates after exposure of the fovea to laser radiation .
	manualset3
143363	6	409033	5	NULL	NULL	0	NULL	nonhuman primates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of experiments was performed to determine the parameters necessary to produce immediate measurable changes in the visual system of nonhuman primates after exposure of the fovea to laser radiation .
	manualset3
143364	8	409033	5	NULL	NULL	NULL	NULL	fovea 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A series of experiments was performed to determine the parameters necessary to produce immediate measurable changes in the visual system of nonhuman primates after exposure of the fovea to laser radiation .
	manualset3
143365	7	409033	5	NULL	NULL	0	NULL	exposure 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of experiments was performed to determine the parameters necessary to produce immediate measurable changes in the visual system of nonhuman primates after exposure of the fovea to laser radiation .
	manualset3
143366	9	409033	5	NULL	NULL	0	NULL	laser radiation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of experiments was performed to determine the parameters necessary to produce immediate measurable changes in the visual system of nonhuman primates after exposure of the fovea to laser radiation .
	manualset3
143367	1	409034	5	NULL	NULL	0	NULL	bundle approach 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The bundle approach recognizes that core clinical interventions , are not always consistently applied across all appropriate patients , the range of interventions within a bundle tackles the problem from a variety of different angles .
	manualset3
143368	2	409034	5	NULL	NULL	0	NULL	core clinical interventions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The bundle approach recognizes that core clinical interventions , are not always consistently applied across all appropriate patients , the range of interventions within a bundle tackles the problem from a variety of different angles .
	manualset3
143369	3	409034	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The bundle approach recognizes that core clinical interventions , are not always consistently applied across all appropriate patients , the range of interventions within a bundle tackles the problem from a variety of different angles .
	manualset3
143370	4	409034	5	NULL	NULL	0	NULL	range 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The bundle approach recognizes that core clinical interventions , are not always consistently applied across all appropriate patients , the range of interventions within a bundle tackles the problem from a variety of different angles .
	manualset3
143371	5	409034	5	NULL	NULL	0	NULL	interventions 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The bundle approach recognizes that core clinical interventions , are not always consistently applied across all appropriate patients , the range of interventions within a bundle tackles the problem from a variety of different angles .
	manualset3
143372	6	409034	5	NULL	NULL	0	NULL	bundle 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The bundle approach recognizes that core clinical interventions , are not always consistently applied across all appropriate patients , the range of interventions within a bundle tackles the problem from a variety of different angles .
	manualset3
143373	7	409034	5	NULL	NULL	0	NULL	problem 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The bundle approach recognizes that core clinical interventions , are not always consistently applied across all appropriate patients , the range of interventions within a bundle tackles the problem from a variety of different angles .
	manualset3
143374	8	409034	5	NULL	NULL	0	NULL	variety 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The bundle approach recognizes that core clinical interventions , are not always consistently applied across all appropriate patients , the range of interventions within a bundle tackles the problem from a variety of different angles .
	manualset3
143375	9	409034	5	NULL	NULL	0	NULL	different angles 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The bundle approach recognizes that core clinical interventions , are not always consistently applied across all appropriate patients , the range of interventions within a bundle tackles the problem from a variety of different angles .
	manualset3
143376	1	409035	5	NULL	NULL	0	NULL	burn surface area percentage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The burn surface area percentage ranged between 2.5 and 70 % ( mean , 22.9 % ) .
	manualset3
143377	2	409035	5	NULL	NULL	0	NULL	2.5 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The burn surface area percentage ranged between 2.5 and 70 % ( mean , 22.9 % ) .
	manualset3
143378	3	409035	5	NULL	NULL	0	NULL	70 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The burn surface area percentage ranged between 2.5 and 70 % ( mean , 22.9 % ) .
	manualset3
143379	4	409035	5	NULL	NULL	0	NULL	mean 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The burn surface area percentage ranged between 2.5 and 70 % ( mean , 22.9 % ) .
	manualset3
143380	5	409035	5	NULL	NULL	0	NULL	22.9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The burn surface area percentage ranged between 2.5 and 70 % ( mean , 22.9 % ) .
	manualset3
143381	1	409036	5	NULL	NULL	0	NULL	bursa of Fabricius 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The bursa of Fabricius presented reduction in the diameters of the follicles , and in the thickness of the cortical and medullary regions .
	manualset3
143382	2	409036	5	NULL	NULL	0	NULL	reduction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The bursa of Fabricius presented reduction in the diameters of the follicles , and in the thickness of the cortical and medullary regions .
	manualset3
143383	3	409036	5	NULL	NULL	0	NULL	diameters 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The bursa of Fabricius presented reduction in the diameters of the follicles , and in the thickness of the cortical and medullary regions .
	manualset3
143384	4	409036	5	NULL	NULL	0	NULL	follicles 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The bursa of Fabricius presented reduction in the diameters of the follicles , and in the thickness of the cortical and medullary regions .
	manualset3
143385	5	409036	5	NULL	NULL	0	NULL	thickness 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The bursa of Fabricius presented reduction in the diameters of the follicles , and in the thickness of the cortical and medullary regions .
	manualset3
143386	6	409036	5	NULL	NULL	0	NULL	cortical regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The bursa of Fabricius presented reduction in the diameters of the follicles , and in the thickness of the cortical and medullary regions .
	manualset3
143387	7	409036	5	NULL	NULL	0	NULL	medullary regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The bursa of Fabricius presented reduction in the diameters of the follicles , and in the thickness of the cortical and medullary regions .
	manualset3
143388	1	409037	5	NULL	NULL	0	NULL	 c-AMP effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The c-AMP effect may be mediated through activation of cyclic AMP-dependent kinase , producing , phosphorylation of the myosin light chain kinase which , according to Adelstein et al. ( 1978 ) , may result in a net dephosphorylation of the myosin light chains and a concomittant inhibition of the contractile response .
	manualset3
143389	2	409037	5	NULL	NULL	0	NULL	activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The c-AMP effect may be mediated through activation of cyclic AMP-dependent kinase , producing , phosphorylation of the myosin light chain kinase which , according to Adelstein et al. ( 1978 ) , may result in a net dephosphorylation of the myosin light chains and a concomittant inhibition of the contractile response .
	manualset3
143390	3	409037	5	NULL	NULL	0	NULL	cyclic AMP-dependent kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The c-AMP effect may be mediated through activation of cyclic AMP-dependent kinase , producing , phosphorylation of the myosin light chain kinase which , according to Adelstein et al. ( 1978 ) , may result in a net dephosphorylation of the myosin light chains and a concomittant inhibition of the contractile response .
	manualset3
143391	4	409037	5	NULL	NULL	0	NULL	phosphorylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The c-AMP effect may be mediated through activation of cyclic AMP-dependent kinase , producing , phosphorylation of the myosin light chain kinase which , according to Adelstein et al. ( 1978 ) , may result in a net dephosphorylation of the myosin light chains and a concomittant inhibition of the contractile response .
	manualset3
143392	5	409037	5	NULL	NULL	0	NULL	myosin light chain kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The c-AMP effect may be mediated through activation of cyclic AMP-dependent kinase , producing , phosphorylation of the myosin light chain kinase which , according to Adelstein et al. ( 1978 ) , may result in a net dephosphorylation of the myosin light chains and a concomittant inhibition of the contractile response .
	manualset3
143393	6	409037	5	NULL	NULL	0	NULL	Adelstein et al. ( 1978 ) 	Citation												NULL		0	NULL	NULL	NULL	NULL	NULL	The c-AMP effect may be mediated through activation of cyclic AMP-dependent kinase , producing , phosphorylation of the myosin light chain kinase which , according to Adelstein et al. ( 1978 ) , may result in a net dephosphorylation of the myosin light chains and a concomittant inhibition of the contractile response .
	manualset3
143394	7	409037	5	NULL	NULL	0	NULL	net dephosphorylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The c-AMP effect may be mediated through activation of cyclic AMP-dependent kinase , producing , phosphorylation of the myosin light chain kinase which , according to Adelstein et al. ( 1978 ) , may result in a net dephosphorylation of the myosin light chains and a concomittant inhibition of the contractile response .
	manualset3
143395	8	409037	5	NULL	NULL	0	NULL	myosin light chains	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The c-AMP effect may be mediated through activation of cyclic AMP-dependent kinase , producing , phosphorylation of the myosin light chain kinase which , according to Adelstein et al. ( 1978 ) , may result in a net dephosphorylation of the myosin light chains and a concomittant inhibition of the contractile response .
	manualset3
143396	9	409037	5	NULL	NULL	0	NULL	concomittant inhibition 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The c-AMP effect may be mediated through activation of cyclic AMP-dependent kinase , producing , phosphorylation of the myosin light chain kinase which , according to Adelstein et al. ( 1978 ) , may result in a net dephosphorylation of the myosin light chains and a concomittant inhibition of the contractile response .
	manualset3
143397	10	409037	5	NULL	NULL	NULL	NULL	contractile response	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The c-AMP effect may be mediated through activation of cyclic AMP-dependent kinase , producing , phosphorylation of the myosin light chain kinase which , according to Adelstein et al. ( 1978 ) , may result in a net dephosphorylation of the myosin light chains and a concomittant inhibition of the contractile response .
	manualset3
143398	1	409038	5	NULL	NULL	0	NULL	cAMP binding protein Epac 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The cAMP binding protein Epac regulates cardiac myofilament function .
	manualset3
143399	2	409038	5	NULL	NULL	0	NULL	cardiac myofilament function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cAMP binding protein Epac regulates cardiac myofilament function .
	manualset3
143400	1	409039	5	NULL	NULL	0	NULL	calcium paradox phenomenon 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The calcium paradox phenomenon : a flow rate and volume response study of calcium-free perfusion .
	manualset3
143401	2	409039	5	NULL	NULL	0	NULL	flow rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The calcium paradox phenomenon : a flow rate and volume response study of calcium-free perfusion .
	manualset3
143402	3	409039	5	NULL	NULL	0	NULL	volume response study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The calcium paradox phenomenon : a flow rate and volume response study of calcium-free perfusion .
	manualset3
143403	4	409039	5	NULL	NULL	0	NULL	calcium-free perfusion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The calcium paradox phenomenon : a flow rate and volume response study of calcium-free perfusion .
	manualset3
143404	1	409040	5	NULL	NULL	0	NULL	calculation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The calculation of entropy gives a precise idea of the degree of order of a phyllotactic system .
	manualset3
143405	2	409040	5	NULL	NULL	0	NULL	entropy 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The calculation of entropy gives a precise idea of the degree of order of a phyllotactic system .
	manualset3
143406	3	409040	5	NULL	NULL	NULL	NULL	idea 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The calculation of entropy gives a precise idea of the degree of order of a phyllotactic system .
	manualset3
143407	4	409040	5	NULL	NULL	0	NULL	degree of order 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The calculation of entropy gives a precise idea of the degree of order of a phyllotactic system .
	manualset3
143408	5	409040	5	NULL	NULL	0	NULL	phyllotactic system	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The calculation of entropy gives a precise idea of the degree of order of a phyllotactic system .
	manualset3
143409	1	409041	5	NULL	NULL	0	NULL	calibration graphs	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The calibration graphs were linear in the range of 2-100 ng mL ( -1 ) with the square of the correlation coefficient R2 ) 0.991 and detection limits were between 0.57 and 1.82 ng mL ( -1 ) .
	manualset3
143410	2	409041	5	NULL	NULL	0	NULL	range 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The calibration graphs were linear in the range of 2-100 ng mL ( -1 ) with the square of the correlation coefficient R2 ) 0.991 and detection limits were between 0.57 and 1.82 ng mL ( -1 ) .
	manualset3
143411	3	409041	5	NULL	NULL	0	NULL	2-100 ng mL ( -1 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The calibration graphs were linear in the range of 2-100 ng mL ( -1 ) with the square of the correlation coefficient R2 ) 0.991 and detection limits were between 0.57 and 1.82 ng mL ( -1 ) .
	manualset3
143412	4	409041	5	NULL	NULL	0	NULL	square of the correlation coefficient R2 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The calibration graphs were linear in the range of 2-100 ng mL ( -1 ) with the square of the correlation coefficient R2 ) 0.991 and detection limits were between 0.57 and 1.82 ng mL ( -1 ) .
	manualset3
143413	5	409041	5	NULL	NULL	0	NULL	0.991	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The calibration graphs were linear in the range of 2-100 ng mL ( -1 ) with the square of the correlation coefficient R2 ) 0.991 and detection limits were between 0.57 and 1.82 ng mL ( -1 ) .
	manualset3
143414	6	409041	5	NULL	NULL	0	NULL	detection limits	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The calibration graphs were linear in the range of 2-100 ng mL ( -1 ) with the square of the correlation coefficient R2 ) 0.991 and detection limits were between 0.57 and 1.82 ng mL ( -1 ) .
	manualset3
143415	7	409041	5	NULL	NULL	0	NULL	0.57  ng mL ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The calibration graphs were linear in the range of 2-100 ng mL ( -1 ) with the square of the correlation coefficient R2 ) 0.991 and detection limits were between 0.57 and 1.82 ng mL ( -1 ) .
	manualset3
143416	8	409041	5	NULL	NULL	0	NULL	1.82 ng mL ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The calibration graphs were linear in the range of 2-100 ng mL ( -1 ) with the square of the correlation coefficient R2 ) 0.991 and detection limits were between 0.57 and 1.82 ng mL ( -1 ) .
	manualset3
143417	1	409042	5	NULL	NULL	0	NULL	campaign 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The campaign was judged not be be cost-effective , and lack of integration with other services , especially expansion of clinic facilities and staff , led to early cancellation .
	manualset3
143418	2	409042	5	NULL	NULL	0	NULL	integration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The campaign was judged not be be cost-effective , and lack of integration with other services , especially expansion of clinic facilities and staff , led to early cancellation .
	manualset3
143419	3	409042	5	NULL	NULL	0	NULL	other services	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The campaign was judged not be be cost-effective , and lack of integration with other services , especially expansion of clinic facilities and staff , led to early cancellation .
	manualset3
143420	4	409042	5	NULL	NULL	0	NULL	expansion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The campaign was judged not be be cost-effective , and lack of integration with other services , especially expansion of clinic facilities and staff , led to early cancellation .
	manualset3
143421	5	409042	5	NULL	NULL	0	NULL	clinic facilities	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The campaign was judged not be be cost-effective , and lack of integration with other services , especially expansion of clinic facilities and staff , led to early cancellation .
	manualset3
143422	6	409042	5	NULL	NULL	0	NULL	staff 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The campaign was judged not be be cost-effective , and lack of integration with other services , especially expansion of clinic facilities and staff , led to early cancellation .
	manualset3
143423	7	409042	5	NULL	NULL	0	NULL	cancellation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The campaign was judged not be be cost-effective , and lack of integration with other services , especially expansion of clinic facilities and staff , led to early cancellation .
	manualset3
143424	1	409043	5	NULL	NULL	0	NULL	camptothecin derivative irinotecan ( CPT-11 )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The camptothecin derivative irinotecan ( CPT-11 ) has been shown to possess antitumor activity in phase II trials for patients with carcinoma of the lung , cervix , ovary , colon , or rectum and for patients with non-Hodgkin 's lymphoma .
	manualset3
143425	2	409043	5	NULL	NULL	0	NULL	antitumor activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The camptothecin derivative irinotecan ( CPT-11 ) has been shown to possess antitumor activity in phase II trials for patients with carcinoma of the lung , cervix , ovary , colon , or rectum and for patients with non-Hodgkin 's lymphoma .
	manualset3
143426	3	409043	5	NULL	NULL	0	NULL	phase II trials 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The camptothecin derivative irinotecan ( CPT-11 ) has been shown to possess antitumor activity in phase II trials for patients with carcinoma of the lung , cervix , ovary , colon , or rectum and for patients with non-Hodgkin 's lymphoma .
	manualset3
143427	4	409043	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The camptothecin derivative irinotecan ( CPT-11 ) has been shown to possess antitumor activity in phase II trials for patients with carcinoma of the lung , cervix , ovary , colon , or rectum and for patients with non-Hodgkin 's lymphoma .
	manualset3
143428	5	409043	5	NULL	NULL	0	NULL	carcinoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The camptothecin derivative irinotecan ( CPT-11 ) has been shown to possess antitumor activity in phase II trials for patients with carcinoma of the lung , cervix , ovary , colon , or rectum and for patients with non-Hodgkin 's lymphoma .
	manualset3
143429	6	409043	5	NULL	NULL	0	NULL	lung 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The camptothecin derivative irinotecan ( CPT-11 ) has been shown to possess antitumor activity in phase II trials for patients with carcinoma of the lung , cervix , ovary , colon , or rectum and for patients with non-Hodgkin 's lymphoma .
	manualset3
143430	7	409043	5	NULL	NULL	0	NULL	cervix 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The camptothecin derivative irinotecan ( CPT-11 ) has been shown to possess antitumor activity in phase II trials for patients with carcinoma of the lung , cervix , ovary , colon , or rectum and for patients with non-Hodgkin 's lymphoma .
	manualset3
143431	8	409043	5	NULL	NULL	0	NULL	ovary 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The camptothecin derivative irinotecan ( CPT-11 ) has been shown to possess antitumor activity in phase II trials for patients with carcinoma of the lung , cervix , ovary , colon , or rectum and for patients with non-Hodgkin 's lymphoma .
	manualset3
143432	9	409043	5	NULL	NULL	0	NULL	colon 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The camptothecin derivative irinotecan ( CPT-11 ) has been shown to possess antitumor activity in phase II trials for patients with carcinoma of the lung , cervix , ovary , colon , or rectum and for patients with non-Hodgkin 's lymphoma .
	manualset3
143433	10	409043	5	NULL	NULL	0	NULL	rectum 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The camptothecin derivative irinotecan ( CPT-11 ) has been shown to possess antitumor activity in phase II trials for patients with carcinoma of the lung , cervix , ovary , colon , or rectum and for patients with non-Hodgkin 's lymphoma .
	manualset3
143434	11	409043	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The camptothecin derivative irinotecan ( CPT-11 ) has been shown to possess antitumor activity in phase II trials for patients with carcinoma of the lung , cervix , ovary , colon , or rectum and for patients with non-Hodgkin 's lymphoma .
	manualset3
143435	12	409043	5	NULL	NULL	0	NULL	non-Hodgkin 's lymphoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The camptothecin derivative irinotecan ( CPT-11 ) has been shown to possess antitumor activity in phase II trials for patients with carcinoma of the lung , cervix , ovary , colon , or rectum and for patients with non-Hodgkin 's lymphoma .
	manualset3
143436	1	409044	5	NULL	NULL	0	NULL	canonical Wnt pathway 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The canonical Wnt pathway was not affected by SFRP2 in endothelial cells ; however , a component of the noncanonical Wnt/Ca2 + pathway was affected by SFRP2 as shown by an increase in NFATc3 in the nuclear fraction of SFRP2-treated endothelial cells .
	manualset3
143437	2	409044	5	NULL	NULL	0	NULL	SFRP2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The canonical Wnt pathway was not affected by SFRP2 in endothelial cells ; however , a component of the noncanonical Wnt/Ca2 + pathway was affected by SFRP2 as shown by an increase in NFATc3 in the nuclear fraction of SFRP2-treated endothelial cells .
	manualset3
143438	3	409044	5	NULL	NULL	0	NULL	endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The canonical Wnt pathway was not affected by SFRP2 in endothelial cells ; however , a component of the noncanonical Wnt/Ca2 + pathway was affected by SFRP2 as shown by an increase in NFATc3 in the nuclear fraction of SFRP2-treated endothelial cells .
	manualset3
143439	4	409044	5	NULL	NULL	0	NULL	component 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The canonical Wnt pathway was not affected by SFRP2 in endothelial cells ; however , a component of the noncanonical Wnt/Ca2 + pathway was affected by SFRP2 as shown by an increase in NFATc3 in the nuclear fraction of SFRP2-treated endothelial cells .
	manualset3
143440	5	409044	5	NULL	NULL	0	NULL	noncanonical Wnt/Ca2 + pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The canonical Wnt pathway was not affected by SFRP2 in endothelial cells ; however , a component of the noncanonical Wnt/Ca2 + pathway was affected by SFRP2 as shown by an increase in NFATc3 in the nuclear fraction of SFRP2-treated endothelial cells .
	manualset3
143441	6	409044	5	NULL	NULL	0	NULL	SFRP2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The canonical Wnt pathway was not affected by SFRP2 in endothelial cells ; however , a component of the noncanonical Wnt/Ca2 + pathway was affected by SFRP2 as shown by an increase in NFATc3 in the nuclear fraction of SFRP2-treated endothelial cells .
	manualset3
143442	7	409044	5	NULL	NULL	0	NULL	NFATc3 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The canonical Wnt pathway was not affected by SFRP2 in endothelial cells ; however , a component of the noncanonical Wnt/Ca2 + pathway was affected by SFRP2 as shown by an increase in NFATc3 in the nuclear fraction of SFRP2-treated endothelial cells .
	manualset3
143443	8	409044	5	NULL	NULL	0	NULL	nuclear fraction 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The canonical Wnt pathway was not affected by SFRP2 in endothelial cells ; however , a component of the noncanonical Wnt/Ca2 + pathway was affected by SFRP2 as shown by an increase in NFATc3 in the nuclear fraction of SFRP2-treated endothelial cells .
	manualset3
143444	9	409044	5	NULL	NULL	0	NULL	SFRP2-treated endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The canonical Wnt pathway was not affected by SFRP2 in endothelial cells ; however , a component of the noncanonical Wnt/Ca2 + pathway was affected by SFRP2 as shown by an increase in NFATc3 in the nuclear fraction of SFRP2-treated endothelial cells .
	manualset3
143445	1	409045	5	NULL	NULL	0	NULL	canton Thurgau	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The canton Thurgau became the most dangerous region in Switzerland for TBE during the last ten years .
	manualset3
143446	2	409045	5	NULL	NULL	0	NULL	region 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The canton Thurgau became the most dangerous region in Switzerland for TBE during the last ten years .
	manualset3
143447	3	409045	5	NULL	NULL	0	NULL	Switzerland 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The canton Thurgau became the most dangerous region in Switzerland for TBE during the last ten years .
	manualset3
143448	4	409045	5	NULL	NULL	0	NULL	TBE 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The canton Thurgau became the most dangerous region in Switzerland for TBE during the last ten years .
	manualset3
143449	5	409045	5	NULL	NULL	0	NULL	ten years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The canton Thurgau became the most dangerous region in Switzerland for TBE during the last ten years .
	manualset3
143450	1	409046	5	NULL	NULL	0	NULL	capability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The capability of seven recombinant human P-450s to hydroxylate salicylate demonstrated that P-450 2E1 and 3A4 contributed to 2 , 5-DHBA formation in approximately equal proportions .
	manualset3
143451	2	409046	5	NULL	NULL	0	NULL	seven	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The capability of seven recombinant human P-450s to hydroxylate salicylate demonstrated that P-450 2E1 and 3A4 contributed to 2 , 5-DHBA formation in approximately equal proportions .
	manualset3
143452	3	409046	5	NULL	NULL	0	NULL	recombinant human P-450s	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The capability of seven recombinant human P-450s to hydroxylate salicylate demonstrated that P-450 2E1 and 3A4 contributed to 2 , 5-DHBA formation in approximately equal proportions .
	manualset3
143453	4	409046	5	NULL	NULL	0	NULL	hydroxylate salicylate 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The capability of seven recombinant human P-450s to hydroxylate salicylate demonstrated that P-450 2E1 and 3A4 contributed to 2 , 5-DHBA formation in approximately equal proportions .
	manualset3
143454	5	409046	5	NULL	NULL	0	NULL	 P-450 2E1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The capability of seven recombinant human P-450s to hydroxylate salicylate demonstrated that P-450 2E1 and 3A4 contributed to 2 , 5-DHBA formation in approximately equal proportions .
	manualset3
143455	6	409046	5	NULL	NULL	0	NULL	 P-450 3A4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The capability of seven recombinant human P-450s to hydroxylate salicylate demonstrated that P-450 2E1 and 3A4 contributed to 2 , 5-DHBA formation in approximately equal proportions .
	manualset3
143456	7	409046	5	NULL	NULL	0	NULL	2 , 5-DHBA formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The capability of seven recombinant human P-450s to hydroxylate salicylate demonstrated that P-450 2E1 and 3A4 contributed to 2 , 5-DHBA formation in approximately equal proportions .
	manualset3
143457	8	409046	5	NULL	NULL	0	NULL	equal proportions	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The capability of seven recombinant human P-450s to hydroxylate salicylate demonstrated that P-450 2E1 and 3A4 contributed to 2 , 5-DHBA formation in approximately equal proportions .
	manualset3
143458	1	409047	5	NULL	NULL	0	NULL	capability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The capability to modify the biochemistry of synapses as well as the growth and change in terms of rewiring of synapses , dendritic branching and glial cell proliferation via the dialogue of synapses and genes , results in specific changes in neuronal connectivity and function .
	manualset3
143459	2	409047	5	NULL	NULL	NULL	NULL	biochemistry 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The capability to modify the biochemistry of synapses as well as the growth and change in terms of rewiring of synapses , dendritic branching and glial cell proliferation via the dialogue of synapses and genes , results in specific changes in neuronal connectivity and function .
	manualset3
143460	3	409047	5	NULL	NULL	0	NULL	synapses 	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The capability to modify the biochemistry of synapses as well as the growth and change in terms of rewiring of synapses , dendritic branching and glial cell proliferation via the dialogue of synapses and genes , results in specific changes in neuronal connectivity and function .
	manualset3
143461	4	409047	5	NULL	NULL	0	NULL	growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The capability to modify the biochemistry of synapses as well as the growth and change in terms of rewiring of synapses , dendritic branching and glial cell proliferation via the dialogue of synapses and genes , results in specific changes in neuronal connectivity and function .
	manualset3
143462	5	409047	5	NULL	NULL	0	NULL	change 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The capability to modify the biochemistry of synapses as well as the growth and change in terms of rewiring of synapses , dendritic branching and glial cell proliferation via the dialogue of synapses and genes , results in specific changes in neuronal connectivity and function .
	manualset3
143463	6	409047	5	NULL	NULL	0	NULL	synapses 	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The capability to modify the biochemistry of synapses as well as the growth and change in terms of rewiring of synapses , dendritic branching and glial cell proliferation via the dialogue of synapses and genes , results in specific changes in neuronal connectivity and function .
	manualset3
143464	7	409047	5	NULL	NULL	0	NULL	dendritic branching 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The capability to modify the biochemistry of synapses as well as the growth and change in terms of rewiring of synapses , dendritic branching and glial cell proliferation via the dialogue of synapses and genes , results in specific changes in neuronal connectivity and function .
	manualset3
143465	8	409047	5	NULL	NULL	0	NULL	glial cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The capability to modify the biochemistry of synapses as well as the growth and change in terms of rewiring of synapses , dendritic branching and glial cell proliferation via the dialogue of synapses and genes , results in specific changes in neuronal connectivity and function .
	manualset3
143466	9	409047	5	NULL	NULL	0	NULL	synapses 	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The capability to modify the biochemistry of synapses as well as the growth and change in terms of rewiring of synapses , dendritic branching and glial cell proliferation via the dialogue of synapses and genes , results in specific changes in neuronal connectivity and function .
	manualset3
143467	10	409047	5	NULL	NULL	0	NULL	genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The capability to modify the biochemistry of synapses as well as the growth and change in terms of rewiring of synapses , dendritic branching and glial cell proliferation via the dialogue of synapses and genes , results in specific changes in neuronal connectivity and function .
	manualset3
143468	11	409047	5	NULL	NULL	0	NULL	specific changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The capability to modify the biochemistry of synapses as well as the growth and change in terms of rewiring of synapses , dendritic branching and glial cell proliferation via the dialogue of synapses and genes , results in specific changes in neuronal connectivity and function .
	manualset3
143469	12	409047	5	NULL	NULL	0	NULL	neuronal connectivity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The capability to modify the biochemistry of synapses as well as the growth and change in terms of rewiring of synapses , dendritic branching and glial cell proliferation via the dialogue of synapses and genes , results in specific changes in neuronal connectivity and function .
	manualset3
143470	13	409047	5	NULL	NULL	0	NULL	function 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The capability to modify the biochemistry of synapses as well as the growth and change in terms of rewiring of synapses , dendritic branching and glial cell proliferation via the dialogue of synapses and genes , results in specific changes in neuronal connectivity and function .
	manualset3
147969	14	409047	5	NULL	NULL	0	NULL	dialogue 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The capability to modify the biochemistry of synapses as well as the growth and change in terms of rewiring of synapses , dendritic branching and glial cell proliferation via the dialogue of synapses and genes , results in specific changes in neuronal connectivity and function .
	manualset3
143471	1	409048	5	NULL	NULL	0	NULL	capacity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The capacity for such rearrangement appears to be a key determinant of its ability to inhibit a wide range of serine proteases .
	manualset3
143472	2	409048	5	NULL	NULL	0	NULL	rearrangement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The capacity for such rearrangement appears to be a key determinant of its ability to inhibit a wide range of serine proteases .
	manualset3
143473	3	409048	5	NULL	NULL	0	NULL	determinant 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The capacity for such rearrangement appears to be a key determinant of its ability to inhibit a wide range of serine proteases .
	manualset3
143474	4	409048	5	NULL	NULL	0	NULL	ability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The capacity for such rearrangement appears to be a key determinant of its ability to inhibit a wide range of serine proteases .
	manualset3
143475	5	409048	5	NULL	NULL	0	NULL	wide range 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The capacity for such rearrangement appears to be a key determinant of its ability to inhibit a wide range of serine proteases .
	manualset3
143476	6	409048	5	NULL	NULL	0	NULL	serine proteases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The capacity for such rearrangement appears to be a key determinant of its ability to inhibit a wide range of serine proteases .
	manualset3
143477	1	409049	5	NULL	NULL	0	NULL	series 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of hydrogen bonds connect the IMP-binding pocket to the active site of the large subunit known to function in the phosphorylation of the unstable intermediate , carbamate .
	manualset3
143478	2	409049	5	NULL	NULL	0	NULL	hydrogen bonds 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of hydrogen bonds connect the IMP-binding pocket to the active site of the large subunit known to function in the phosphorylation of the unstable intermediate , carbamate .
	manualset3
143479	3	409049	5	NULL	NULL	0	NULL	IMP-binding pocket	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of hydrogen bonds connect the IMP-binding pocket to the active site of the large subunit known to function in the phosphorylation of the unstable intermediate , carbamate .
	manualset3
143480	4	409049	5	NULL	NULL	0	NULL	active site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of hydrogen bonds connect the IMP-binding pocket to the active site of the large subunit known to function in the phosphorylation of the unstable intermediate , carbamate .
	manualset3
143481	5	409049	5	NULL	NULL	0	NULL	large subunit 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of hydrogen bonds connect the IMP-binding pocket to the active site of the large subunit known to function in the phosphorylation of the unstable intermediate , carbamate .
	manualset3
143482	6	409049	5	NULL	NULL	0	NULL	function 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of hydrogen bonds connect the IMP-binding pocket to the active site of the large subunit known to function in the phosphorylation of the unstable intermediate , carbamate .
	manualset3
143483	7	409049	5	NULL	NULL	0	NULL	phosphorylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of hydrogen bonds connect the IMP-binding pocket to the active site of the large subunit known to function in the phosphorylation of the unstable intermediate , carbamate .
	manualset3
143484	8	409049	5	NULL	NULL	0	NULL	unstable intermediate , carbamate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of hydrogen bonds connect the IMP-binding pocket to the active site of the large subunit known to function in the phosphorylation of the unstable intermediate , carbamate .
	manualset3
143485	1	409050	5	NULL	NULL	0	NULL	carbamino combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The carbamino combination of CO2 with reduced hemoglobin and oxyhemoglobin .
	manualset3
143486	2	409050	5	NULL	NULL	0	NULL	CO2 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The carbamino combination of CO2 with reduced hemoglobin and oxyhemoglobin .
	manualset3
143487	3	409050	5	NULL	NULL	0	NULL	reduced hemoglobin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The carbamino combination of CO2 with reduced hemoglobin and oxyhemoglobin .
	manualset3
143488	4	409050	5	NULL	NULL	0	NULL	oxyhemoglobin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The carbamino combination of CO2 with reduced hemoglobin and oxyhemoglobin .
	manualset3
143489	1	409051	5	NULL	NULL	0	NULL	carbohydrate moiety 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The carbohydrate moiety of band-3 glycoprotein of human erythrocyte membranes .
	manualset3
143490	2	409051	5	NULL	NULL	0	NULL	band-3 glycoprotein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The carbohydrate moiety of band-3 glycoprotein of human erythrocyte membranes .
	manualset3
143491	3	409051	5	NULL	NULL	0	NULL	human erythrocyte membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The carbohydrate moiety of band-3 glycoprotein of human erythrocyte membranes .
	manualset3
143492	1	409052	5	NULL	NULL	0	NULL	carbohydrates 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The carbohydrates were analyzed by anion-exchange chromatography with pulsed amperometric detection and the amino acids by reversed phase chromatography after derivatization with 6-amino-quinolyl-N-hydroxysuccinimidyl carbamate and fluorescence detection .
	manualset3
143493	2	409052	5	NULL	NULL	0	NULL	anion-exchange chromatography 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The carbohydrates were analyzed by anion-exchange chromatography with pulsed amperometric detection and the amino acids by reversed phase chromatography after derivatization with 6-amino-quinolyl-N-hydroxysuccinimidyl carbamate and fluorescence detection .
	manualset3
143494	3	409052	5	NULL	NULL	0	NULL	pulsed amperometric detection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The carbohydrates were analyzed by anion-exchange chromatography with pulsed amperometric detection and the amino acids by reversed phase chromatography after derivatization with 6-amino-quinolyl-N-hydroxysuccinimidyl carbamate and fluorescence detection .
	manualset3
143495	4	409052	5	NULL	NULL	0	NULL	amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The carbohydrates were analyzed by anion-exchange chromatography with pulsed amperometric detection and the amino acids by reversed phase chromatography after derivatization with 6-amino-quinolyl-N-hydroxysuccinimidyl carbamate and fluorescence detection .
	manualset3
143496	5	409052	5	NULL	NULL	0	NULL	reversed phase chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The carbohydrates were analyzed by anion-exchange chromatography with pulsed amperometric detection and the amino acids by reversed phase chromatography after derivatization with 6-amino-quinolyl-N-hydroxysuccinimidyl carbamate and fluorescence detection .
	manualset3
143497	6	409052	5	NULL	NULL	0	NULL	derivatization 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The carbohydrates were analyzed by anion-exchange chromatography with pulsed amperometric detection and the amino acids by reversed phase chromatography after derivatization with 6-amino-quinolyl-N-hydroxysuccinimidyl carbamate and fluorescence detection .
	manualset3
143498	7	409052	5	NULL	NULL	0	NULL	6-amino-quinolyl-N-hydroxysuccinimidyl carbamate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The carbohydrates were analyzed by anion-exchange chromatography with pulsed amperometric detection and the amino acids by reversed phase chromatography after derivatization with 6-amino-quinolyl-N-hydroxysuccinimidyl carbamate and fluorescence detection .
	manualset3
143499	8	409052	5	NULL	NULL	0	NULL	fluorescence detection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The carbohydrates were analyzed by anion-exchange chromatography with pulsed amperometric detection and the amino acids by reversed phase chromatography after derivatization with 6-amino-quinolyl-N-hydroxysuccinimidyl carbamate and fluorescence detection .
	manualset3
143500	1	409053	5	NULL	NULL	0	NULL	carbon material	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The carbon material and energy balances were adequately applied to estimate the carbon-flow distribution .
	manualset3
143501	2	409053	5	NULL	NULL	0	NULL	energy balances 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The carbon material and energy balances were adequately applied to estimate the carbon-flow distribution .
	manualset3
143502	3	409053	5	NULL	NULL	0	NULL	carbon-flow distribution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The carbon material and energy balances were adequately applied to estimate the carbon-flow distribution .
	manualset3
143503	1	409054	5	NULL	NULL	0	NULL	carbonyl-compound-catalyzed nitrosation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The carbonyl-compound-catalyzed nitrosation of amines to form carcinogenic nitrosamines under nonacidic condition is different from the classic nitrosation via acidification of nitrite anion .
	manualset3
143504	2	409054	5	NULL	NULL	0	NULL	amines 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The carbonyl-compound-catalyzed nitrosation of amines to form carcinogenic nitrosamines under nonacidic condition is different from the classic nitrosation via acidification of nitrite anion .
	manualset3
143505	3	409054	5	NULL	NULL	0	NULL	carcinogenic nitrosamines 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The carbonyl-compound-catalyzed nitrosation of amines to form carcinogenic nitrosamines under nonacidic condition is different from the classic nitrosation via acidification of nitrite anion .
	manualset3
143506	4	409054	5	NULL	NULL	0	NULL	nonacidic condition	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The carbonyl-compound-catalyzed nitrosation of amines to form carcinogenic nitrosamines under nonacidic condition is different from the classic nitrosation via acidification of nitrite anion .
	manualset3
143507	5	409054	5	NULL	NULL	0	NULL	classic nitrosation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The carbonyl-compound-catalyzed nitrosation of amines to form carcinogenic nitrosamines under nonacidic condition is different from the classic nitrosation via acidification of nitrite anion .
	manualset3
143508	6	409054	5	NULL	NULL	0	NULL	acidification 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The carbonyl-compound-catalyzed nitrosation of amines to form carcinogenic nitrosamines under nonacidic condition is different from the classic nitrosation via acidification of nitrite anion .
	manualset3
143509	7	409054	5	NULL	NULL	0	NULL	nitrite anion	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The carbonyl-compound-catalyzed nitrosation of amines to form carcinogenic nitrosamines under nonacidic condition is different from the classic nitrosation via acidification of nitrite anion .
	manualset3
143510	1	409055	5	NULL	NULL	0	NULL	cardiomyopathy 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The cardiomyopathy of morbid obesity is characterized by cardiomegaly , left ventricular dilatation , and myocyte hypertrophy in the absence of interstitial fibrosis .
	manualset3
143511	2	409055	5	NULL	NULL	0	NULL	morbid obesity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cardiomyopathy of morbid obesity is characterized by cardiomegaly , left ventricular dilatation , and myocyte hypertrophy in the absence of interstitial fibrosis .
	manualset3
143512	3	409055	5	NULL	NULL	0	NULL	cardiomegaly 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cardiomyopathy of morbid obesity is characterized by cardiomegaly , left ventricular dilatation , and myocyte hypertrophy in the absence of interstitial fibrosis .
	manualset3
143513	4	409055	5	NULL	NULL	0	NULL	left ventricular dilatation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cardiomyopathy of morbid obesity is characterized by cardiomegaly , left ventricular dilatation , and myocyte hypertrophy in the absence of interstitial fibrosis .
	manualset3
143514	5	409055	5	NULL	NULL	0	NULL	myocyte hypertrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cardiomyopathy of morbid obesity is characterized by cardiomegaly , left ventricular dilatation , and myocyte hypertrophy in the absence of interstitial fibrosis .
	manualset3
143515	6	409055	5	NULL	NULL	0	NULL	absence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cardiomyopathy of morbid obesity is characterized by cardiomegaly , left ventricular dilatation , and myocyte hypertrophy in the absence of interstitial fibrosis .
	manualset3
143516	7	409055	5	NULL	NULL	0	NULL	interstitial fibrosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The cardiomyopathy of morbid obesity is characterized by cardiomegaly , left ventricular dilatation , and myocyte hypertrophy in the absence of interstitial fibrosis .
	manualset3
143517	1	409056	5	NULL	NULL	0	NULL	carotid body ( CB ) 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The carotid body ( CB ) plays an important role in the control of breathing and in autonomic control of cardiovascular function .
	manualset3
143518	2	409056	5	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The carotid body ( CB ) plays an important role in the control of breathing and in autonomic control of cardiovascular function .
	manualset3
143519	3	409056	5	NULL	NULL	0	NULL	control 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The carotid body ( CB ) plays an important role in the control of breathing and in autonomic control of cardiovascular function .
	manualset3
143520	4	409056	5	NULL	NULL	0	NULL	breathing 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The carotid body ( CB ) plays an important role in the control of breathing and in autonomic control of cardiovascular function .
	manualset3
143521	5	409056	5	NULL	NULL	0	NULL	autonomic control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The carotid body ( CB ) plays an important role in the control of breathing and in autonomic control of cardiovascular function .
	manualset3
143522	6	409056	5	NULL	NULL	0	NULL	cardiovascular function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The carotid body ( CB ) plays an important role in the control of breathing and in autonomic control of cardiovascular function .
	manualset3
143523	1	409057	5	NULL	NULL	0	NULL	series 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of lithium and sodium complexes with OOO-tridentate bis ( phenolate ) ligands have been synthesized and fully characterized .
	manualset3
143524	2	409057	5	NULL	NULL	0	NULL	lithium 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of lithium and sodium complexes with OOO-tridentate bis ( phenolate ) ligands have been synthesized and fully characterized .
	manualset3
143525	3	409057	5	NULL	NULL	0	NULL	sodium complexes	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of lithium and sodium complexes with OOO-tridentate bis ( phenolate ) ligands have been synthesized and fully characterized .
	manualset3
143526	4	409057	5	NULL	NULL	0	NULL	 OOO-tridentate bis ( phenolate ) ligands	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of lithium and sodium complexes with OOO-tridentate bis ( phenolate ) ligands have been synthesized and fully characterized .
	manualset3
143527	1	409058	5	NULL	NULL	0	NULL	carotid intima-media thickness	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The carotid intima-media thickness was similar between uremic patients and controls .
	manualset3
143528	2	409058	5	NULL	NULL	0	NULL	uremic patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The carotid intima-media thickness was similar between uremic patients and controls .
	manualset3
143529	3	409058	5	NULL	NULL	0	NULL	controls 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The carotid intima-media thickness was similar between uremic patients and controls .
	manualset3
143530	1	409059	5	NULL	NULL	0	NULL	carotids 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The carotids and ophthalmics are densely innervated and are accompanied by thick nerve bundles , suggesting that the nerves preferentially enter the skull along those arteries .
	manualset3
143531	2	409059	5	NULL	NULL	0	NULL	ophthalmics 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The carotids and ophthalmics are densely innervated and are accompanied by thick nerve bundles , suggesting that the nerves preferentially enter the skull along those arteries .
	manualset3
143532	3	409059	5	NULL	NULL	0	NULL	thick nerve bundles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The carotids and ophthalmics are densely innervated and are accompanied by thick nerve bundles , suggesting that the nerves preferentially enter the skull along those arteries .
	manualset3
143533	4	409059	5	NULL	NULL	0	NULL	nerves 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The carotids and ophthalmics are densely innervated and are accompanied by thick nerve bundles , suggesting that the nerves preferentially enter the skull along those arteries .
	manualset3
143534	5	409059	5	NULL	NULL	0	NULL	skull 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The carotids and ophthalmics are densely innervated and are accompanied by thick nerve bundles , suggesting that the nerves preferentially enter the skull along those arteries .
	manualset3
143535	6	409059	5	NULL	NULL	0	NULL	arteries 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The carotids and ophthalmics are densely innervated and are accompanied by thick nerve bundles , suggesting that the nerves preferentially enter the skull along those arteries .
	manualset3
143536	1	409060	5	NULL	NULL	0	NULL	carrier-envelope phase ( CEP )	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The carrier-envelope phase ( CEP ) of the pulse , which in the multi-cycle regime does not play any control role , is shown here to be a new effective control parameter that its effect is highly sensitive to the spectral position of the ultrabroad spectrum .
	manualset3
143537	2	409060	5	NULL	NULL	0	NULL	pulse 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The carrier-envelope phase ( CEP ) of the pulse , which in the multi-cycle regime does not play any control role , is shown here to be a new effective control parameter that its effect is highly sensitive to the spectral position of the ultrabroad spectrum .
	manualset3
143538	3	409060	5	NULL	NULL	0	NULL	multi-cycle regime	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The carrier-envelope phase ( CEP ) of the pulse , which in the multi-cycle regime does not play any control role , is shown here to be a new effective control parameter that its effect is highly sensitive to the spectral position of the ultrabroad spectrum .
	manualset3
143539	4	409060	5	NULL	NULL	0	NULL	control role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The carrier-envelope phase ( CEP ) of the pulse , which in the multi-cycle regime does not play any control role , is shown here to be a new effective control parameter that its effect is highly sensitive to the spectral position of the ultrabroad spectrum .
	manualset3
143540	5	409060	5	NULL	NULL	0	NULL	effective control parameter 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The carrier-envelope phase ( CEP ) of the pulse , which in the multi-cycle regime does not play any control role , is shown here to be a new effective control parameter that its effect is highly sensitive to the spectral position of the ultrabroad spectrum .
	manualset3
143541	6	409060	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The carrier-envelope phase ( CEP ) of the pulse , which in the multi-cycle regime does not play any control role , is shown here to be a new effective control parameter that its effect is highly sensitive to the spectral position of the ultrabroad spectrum .
	manualset3
143542	7	409060	5	NULL	NULL	0	NULL	spectral position	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The carrier-envelope phase ( CEP ) of the pulse , which in the multi-cycle regime does not play any control role , is shown here to be a new effective control parameter that its effect is highly sensitive to the spectral position of the ultrabroad spectrum .
	manualset3
143543	8	409060	5	NULL	NULL	0	NULL	ultrabroad spectrum	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The carrier-envelope phase ( CEP ) of the pulse , which in the multi-cycle regime does not play any control role , is shown here to be a new effective control parameter that its effect is highly sensitive to the spectral position of the ultrabroad spectrum .
	manualset3
143544	1	409061	5	NULL	NULL	0	NULL	carrier transport 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The carrier transport to the metal anode is likely enhanced through shallow gap states in the MoO ( x ) layer .
	manualset3
143545	2	409061	5	NULL	NULL	0	NULL	metal anode	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The carrier transport to the metal anode is likely enhanced through shallow gap states in the MoO ( x ) layer .
	manualset3
143546	3	409061	5	NULL	NULL	0	NULL	shallow gap states	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The carrier transport to the metal anode is likely enhanced through shallow gap states in the MoO ( x ) layer .
	manualset3
143547	4	409061	5	NULL	NULL	0	NULL	MoO ( x ) layer 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The carrier transport to the metal anode is likely enhanced through shallow gap states in the MoO ( x ) layer .
	manualset3
143548	1	409062	5	NULL	NULL	0	NULL	case histories	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The case histories of six patients are presented where the diagnosis of carcinoma of the esophagus and the stomach was made at the same time by barium studies .
	manualset3
143549	2	409062	5	NULL	NULL	0	NULL	six patients	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The case histories of six patients are presented where the diagnosis of carcinoma of the esophagus and the stomach was made at the same time by barium studies .
	manualset3
143550	3	409062	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The case histories of six patients are presented where the diagnosis of carcinoma of the esophagus and the stomach was made at the same time by barium studies .
	manualset3
143551	4	409062	5	NULL	NULL	0	NULL	carcinoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The case histories of six patients are presented where the diagnosis of carcinoma of the esophagus and the stomach was made at the same time by barium studies .
	manualset3
143552	5	409062	5	NULL	NULL	0	NULL	esophagus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The case histories of six patients are presented where the diagnosis of carcinoma of the esophagus and the stomach was made at the same time by barium studies .
	manualset3
143553	6	409062	5	NULL	NULL	0	NULL	stomach 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The case histories of six patients are presented where the diagnosis of carcinoma of the esophagus and the stomach was made at the same time by barium studies .
	manualset3
143554	7	409062	5	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The case histories of six patients are presented where the diagnosis of carcinoma of the esophagus and the stomach was made at the same time by barium studies .
	manualset3
143555	8	409062	5	NULL	NULL	0	NULL	barium studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The case histories of six patients are presented where the diagnosis of carcinoma of the esophagus and the stomach was made at the same time by barium studies .
	manualset3
143556	1	409063	5	NULL	NULL	0	NULL	case 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The case may illustrate a role for the thalamus in regulating ventilation , but another small infarct not visible on MRI also could be responsible .
	manualset3
143557	2	409063	5	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The case may illustrate a role for the thalamus in regulating ventilation , but another small infarct not visible on MRI also could be responsible .
	manualset3
143558	3	409063	5	NULL	NULL	0	NULL	thalamus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The case may illustrate a role for the thalamus in regulating ventilation , but another small infarct not visible on MRI also could be responsible .
	manualset3
143559	4	409063	5	NULL	NULL	0	NULL	ventilation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The case may illustrate a role for the thalamus in regulating ventilation , but another small infarct not visible on MRI also could be responsible .
	manualset3
143560	5	409063	5	NULL	NULL	0	NULL	small infarct	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The case may illustrate a role for the thalamus in regulating ventilation , but another small infarct not visible on MRI also could be responsible .
	manualset3
143561	6	409063	5	NULL	NULL	0	NULL	MRI 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The case may illustrate a role for the thalamus in regulating ventilation , but another small infarct not visible on MRI also could be responsible .
	manualset3
143562	1	409064	5	NULL	NULL	0	NULL	case 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of Retacrit , one of the biosimilar epoetines , is being discussed as an example of the challenges encountered when assessing the bioequivalence of therapeutic proteins .
	manualset3
143563	2	409064	5	NULL	NULL	0	NULL	Retacrit 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of Retacrit , one of the biosimilar epoetines , is being discussed as an example of the challenges encountered when assessing the bioequivalence of therapeutic proteins .
	manualset3
143564	3	409064	5	NULL	NULL	0	NULL	biosimilar epoetines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of Retacrit , one of the biosimilar epoetines , is being discussed as an example of the challenges encountered when assessing the bioequivalence of therapeutic proteins .
	manualset3
143565	4	409064	5	NULL	NULL	0	NULL	example 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of Retacrit , one of the biosimilar epoetines , is being discussed as an example of the challenges encountered when assessing the bioequivalence of therapeutic proteins .
	manualset3
143566	5	409064	5	NULL	NULL	0	NULL	challenges 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of Retacrit , one of the biosimilar epoetines , is being discussed as an example of the challenges encountered when assessing the bioequivalence of therapeutic proteins .
	manualset3
143567	6	409064	5	NULL	NULL	0	NULL	bioequivalence 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of Retacrit , one of the biosimilar epoetines , is being discussed as an example of the challenges encountered when assessing the bioequivalence of therapeutic proteins .
	manualset3
143568	7	409064	5	NULL	NULL	0	NULL	therapeutic proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of Retacrit , one of the biosimilar epoetines , is being discussed as an example of the challenges encountered when assessing the bioequivalence of therapeutic proteins .
	manualset3
143569	1	409065	5	NULL	NULL	0	NULL	series 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of nanoindentation tests were performed on various locations of cellulosic thecal plates isolated from the dinoflagellates Alexandrium catenella and Lingulodinium polyedrum .
	manualset3
143570	2	409065	5	NULL	NULL	0	NULL	nanoindentation tests	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of nanoindentation tests were performed on various locations of cellulosic thecal plates isolated from the dinoflagellates Alexandrium catenella and Lingulodinium polyedrum .
	manualset3
143571	3	409065	5	NULL	NULL	0	NULL	various locations 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of nanoindentation tests were performed on various locations of cellulosic thecal plates isolated from the dinoflagellates Alexandrium catenella and Lingulodinium polyedrum .
	manualset3
143572	4	409065	5	NULL	NULL	0	NULL	cellulosic thecal plates	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of nanoindentation tests were performed on various locations of cellulosic thecal plates isolated from the dinoflagellates Alexandrium catenella and Lingulodinium polyedrum .
	manualset3
143573	5	409065	5	NULL	NULL	0	NULL	dinoflagellate Alexandrium catenella 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of nanoindentation tests were performed on various locations of cellulosic thecal plates isolated from the dinoflagellates Alexandrium catenella and Lingulodinium polyedrum .
	manualset3
143574	6	409065	5	NULL	NULL	0	NULL	dinoflagellate Lingulodinium polyedrum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of nanoindentation tests were performed on various locations of cellulosic thecal plates isolated from the dinoflagellates Alexandrium catenella and Lingulodinium polyedrum .
	manualset3
143575	1	409066	5	NULL	NULL	0	NULL	case 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of a 15-year-old boy who developed pulmonary zygomycosis while on chemotherapy for acute lymphoblastic leukemia , and who survived for 11 months with oral fluconazole therapy alone , is supportive of this proposal .
	manualset3
143576	2	409066	5	NULL	NULL	0	NULL	15-year-old boy	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of a 15-year-old boy who developed pulmonary zygomycosis while on chemotherapy for acute lymphoblastic leukemia , and who survived for 11 months with oral fluconazole therapy alone , is supportive of this proposal .
	manualset3
143577	3	409066	5	NULL	NULL	0	NULL	pulmonary zygomycosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of a 15-year-old boy who developed pulmonary zygomycosis while on chemotherapy for acute lymphoblastic leukemia , and who survived for 11 months with oral fluconazole therapy alone , is supportive of this proposal .
	manualset3
143578	4	409066	5	NULL	NULL	0	NULL	chemotherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of a 15-year-old boy who developed pulmonary zygomycosis while on chemotherapy for acute lymphoblastic leukemia , and who survived for 11 months with oral fluconazole therapy alone , is supportive of this proposal .
	manualset3
143579	5	409066	5	NULL	NULL	0	NULL	acute lymphoblastic leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of a 15-year-old boy who developed pulmonary zygomycosis while on chemotherapy for acute lymphoblastic leukemia , and who survived for 11 months with oral fluconazole therapy alone , is supportive of this proposal .
	manualset3
143580	6	409066	5	NULL	NULL	0	NULL	11 months 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of a 15-year-old boy who developed pulmonary zygomycosis while on chemotherapy for acute lymphoblastic leukemia , and who survived for 11 months with oral fluconazole therapy alone , is supportive of this proposal .
	manualset3
143581	7	409066	5	NULL	NULL	0	NULL	oral fluconazole therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of a 15-year-old boy who developed pulmonary zygomycosis while on chemotherapy for acute lymphoblastic leukemia , and who survived for 11 months with oral fluconazole therapy alone , is supportive of this proposal .
	manualset3
143582	8	409066	5	NULL	NULL	0	NULL	proposal 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of a 15-year-old boy who developed pulmonary zygomycosis while on chemotherapy for acute lymphoblastic leukemia , and who survived for 11 months with oral fluconazole therapy alone , is supportive of this proposal .
	manualset3
143583	1	409067	5	NULL	NULL	0	NULL	case 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of a 7-year-old girl , born from a monochorionic biamniotic pregnancy ( with healthy male twin ) is presented .
	manualset3
143584	2	409067	5	NULL	NULL	0	NULL	7-year-old girl 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of a 7-year-old girl , born from a monochorionic biamniotic pregnancy ( with healthy male twin ) is presented .
	manualset3
143585	3	409067	5	NULL	NULL	0	NULL	monochorionic biamniotic pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of a 7-year-old girl , born from a monochorionic biamniotic pregnancy ( with healthy male twin ) is presented .
	manualset3
143586	4	409067	5	NULL	NULL	0	NULL	healthy male twin	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of a 7-year-old girl , born from a monochorionic biamniotic pregnancy ( with healthy male twin ) is presented .
	manualset3
143587	1	409068	5	NULL	NULL	0	NULL	case 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of complete necrosis was related to the frequency of the catheter arriving at the tumor , to the types of embolizing drug , and to the morphopathologic features of the tumor .
	manualset3
143588	2	409068	5	NULL	NULL	0	NULL	complete necrosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of complete necrosis was related to the frequency of the catheter arriving at the tumor , to the types of embolizing drug , and to the morphopathologic features of the tumor .
	manualset3
143589	3	409068	5	NULL	NULL	0	NULL	frequency 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of complete necrosis was related to the frequency of the catheter arriving at the tumor , to the types of embolizing drug , and to the morphopathologic features of the tumor .
	manualset3
143590	4	409068	5	NULL	NULL	0	NULL	catheter 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of complete necrosis was related to the frequency of the catheter arriving at the tumor , to the types of embolizing drug , and to the morphopathologic features of the tumor .
	manualset3
143591	5	409068	5	NULL	NULL	0	NULL	tumor 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of complete necrosis was related to the frequency of the catheter arriving at the tumor , to the types of embolizing drug , and to the morphopathologic features of the tumor .
	manualset3
143592	6	409068	5	NULL	NULL	0	NULL	types 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of complete necrosis was related to the frequency of the catheter arriving at the tumor , to the types of embolizing drug , and to the morphopathologic features of the tumor .
	manualset3
143593	7	409068	5	NULL	NULL	0	NULL	embolizing drug 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of complete necrosis was related to the frequency of the catheter arriving at the tumor , to the types of embolizing drug , and to the morphopathologic features of the tumor .
	manualset3
143594	8	409068	5	NULL	NULL	0	NULL	morphopathologic features 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of complete necrosis was related to the frequency of the catheter arriving at the tumor , to the types of embolizing drug , and to the morphopathologic features of the tumor .
	manualset3
143595	9	409068	5	NULL	NULL	0	NULL	tumor 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of complete necrosis was related to the frequency of the catheter arriving at the tumor , to the types of embolizing drug , and to the morphopathologic features of the tumor .
	manualset3
143596	1	409069	5	NULL	NULL	0	NULL	case 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The case was presumed to be GIN associated with UTI or hypersensitivity to medication .
	manualset3
143597	2	409069	5	NULL	NULL	0	NULL	GIN 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The case was presumed to be GIN associated with UTI or hypersensitivity to medication .
	manualset3
143598	3	409069	5	NULL	NULL	0	NULL	UTI 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The case was presumed to be GIN associated with UTI or hypersensitivity to medication .
	manualset3
143599	4	409069	5	NULL	NULL	0	NULL	hypersensitivity to medication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The case was presumed to be GIN associated with UTI or hypersensitivity to medication .
	manualset3
143600	1	409070	5	NULL	NULL	0	NULL	cat iris contraction data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The cat iris contraction data were well correlated with other FP-receptor-mediated signal-transduction processes , including FP-receptor binding in bovine corpus luteum ( r = 0.86 ) , FP-receptor binding in human iris ( r = 0.61 ) , phosphoinositide ( PI ) hydrolysis in human ciliary muscle and trabecular meshwork cells ( r = 0.77 - 0.86 ) , PI turnover in rat and mouse cells ( r = 0.73 - 0.76 ) and via cloned human FP-receptor ( r = 0.9 ) , and rat uterus contraction ( r = 0.84 ) .
	manualset3
143601	2	409070	5	NULL	NULL	0	NULL	FP-receptor-mediated signal-transduction processes 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cat iris contraction data were well correlated with other FP-receptor-mediated signal-transduction processes , including FP-receptor binding in bovine corpus luteum ( r = 0.86 ) , FP-receptor binding in human iris ( r = 0.61 ) , phosphoinositide ( PI ) hydrolysis in human ciliary muscle and trabecular meshwork cells ( r = 0.77 - 0.86 ) , PI turnover in rat and mouse cells ( r = 0.73 - 0.76 ) and via cloned human FP-receptor ( r = 0.9 ) , and rat uterus contraction ( r = 0.84 ) .
	manualset3
143602	3	409070	5	NULL	NULL	0	NULL	FP-receptor binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cat iris contraction data were well correlated with other FP-receptor-mediated signal-transduction processes , including FP-receptor binding in bovine corpus luteum ( r = 0.86 ) , FP-receptor binding in human iris ( r = 0.61 ) , phosphoinositide ( PI ) hydrolysis in human ciliary muscle and trabecular meshwork cells ( r = 0.77 - 0.86 ) , PI turnover in rat and mouse cells ( r = 0.73 - 0.76 ) and via cloned human FP-receptor ( r = 0.9 ) , and rat uterus contraction ( r = 0.84 ) .
	manualset3
143603	4	409070	5	NULL	NULL	0	NULL	bovine corpus luteum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The cat iris contraction data were well correlated with other FP-receptor-mediated signal-transduction processes , including FP-receptor binding in bovine corpus luteum ( r = 0.86 ) , FP-receptor binding in human iris ( r = 0.61 ) , phosphoinositide ( PI ) hydrolysis in human ciliary muscle and trabecular meshwork cells ( r = 0.77 - 0.86 ) , PI turnover in rat and mouse cells ( r = 0.73 - 0.76 ) and via cloned human FP-receptor ( r = 0.9 ) , and rat uterus contraction ( r = 0.84 ) .
	manualset3
143604	5	409070	5	NULL	NULL	0	NULL	 r = 0.86	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The cat iris contraction data were well correlated with other FP-receptor-mediated signal-transduction processes , including FP-receptor binding in bovine corpus luteum ( r = 0.86 ) , FP-receptor binding in human iris ( r = 0.61 ) , phosphoinositide ( PI ) hydrolysis in human ciliary muscle and trabecular meshwork cells ( r = 0.77 - 0.86 ) , PI turnover in rat and mouse cells ( r = 0.73 - 0.76 ) and via cloned human FP-receptor ( r = 0.9 ) , and rat uterus contraction ( r = 0.84 ) .
	manualset3
143605	6	409070	5	NULL	NULL	0	NULL	FP-receptor binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cat iris contraction data were well correlated with other FP-receptor-mediated signal-transduction processes , including FP-receptor binding in bovine corpus luteum ( r = 0.86 ) , FP-receptor binding in human iris ( r = 0.61 ) , phosphoinositide ( PI ) hydrolysis in human ciliary muscle and trabecular meshwork cells ( r = 0.77 - 0.86 ) , PI turnover in rat and mouse cells ( r = 0.73 - 0.76 ) and via cloned human FP-receptor ( r = 0.9 ) , and rat uterus contraction ( r = 0.84 ) .
	manualset3
143606	7	409070	5	NULL	NULL	0	NULL	human iris	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The cat iris contraction data were well correlated with other FP-receptor-mediated signal-transduction processes , including FP-receptor binding in bovine corpus luteum ( r = 0.86 ) , FP-receptor binding in human iris ( r = 0.61 ) , phosphoinositide ( PI ) hydrolysis in human ciliary muscle and trabecular meshwork cells ( r = 0.77 - 0.86 ) , PI turnover in rat and mouse cells ( r = 0.73 - 0.76 ) and via cloned human FP-receptor ( r = 0.9 ) , and rat uterus contraction ( r = 0.84 ) .
	manualset3
143607	8	409070	5	NULL	NULL	0	NULL	 r = 0.61	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The cat iris contraction data were well correlated with other FP-receptor-mediated signal-transduction processes , including FP-receptor binding in bovine corpus luteum ( r = 0.86 ) , FP-receptor binding in human iris ( r = 0.61 ) , phosphoinositide ( PI ) hydrolysis in human ciliary muscle and trabecular meshwork cells ( r = 0.77 - 0.86 ) , PI turnover in rat and mouse cells ( r = 0.73 - 0.76 ) and via cloned human FP-receptor ( r = 0.9 ) , and rat uterus contraction ( r = 0.84 ) .
	manualset3
143608	9	409070	5	NULL	NULL	0	NULL	phosphoinositide ( PI ) hydrolysis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cat iris contraction data were well correlated with other FP-receptor-mediated signal-transduction processes , including FP-receptor binding in bovine corpus luteum ( r = 0.86 ) , FP-receptor binding in human iris ( r = 0.61 ) , phosphoinositide ( PI ) hydrolysis in human ciliary muscle and trabecular meshwork cells ( r = 0.77 - 0.86 ) , PI turnover in rat and mouse cells ( r = 0.73 - 0.76 ) and via cloned human FP-receptor ( r = 0.9 ) , and rat uterus contraction ( r = 0.84 ) .
	manualset3
143609	10	409070	5	NULL	NULL	0	NULL	human ciliary muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The cat iris contraction data were well correlated with other FP-receptor-mediated signal-transduction processes , including FP-receptor binding in bovine corpus luteum ( r = 0.86 ) , FP-receptor binding in human iris ( r = 0.61 ) , phosphoinositide ( PI ) hydrolysis in human ciliary muscle and trabecular meshwork cells ( r = 0.77 - 0.86 ) , PI turnover in rat and mouse cells ( r = 0.73 - 0.76 ) and via cloned human FP-receptor ( r = 0.9 ) , and rat uterus contraction ( r = 0.84 ) .
	manualset3
143610	11	409070	5	NULL	NULL	0	NULL	trabecular meshwork cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The cat iris contraction data were well correlated with other FP-receptor-mediated signal-transduction processes , including FP-receptor binding in bovine corpus luteum ( r = 0.86 ) , FP-receptor binding in human iris ( r = 0.61 ) , phosphoinositide ( PI ) hydrolysis in human ciliary muscle and trabecular meshwork cells ( r = 0.77 - 0.86 ) , PI turnover in rat and mouse cells ( r = 0.73 - 0.76 ) and via cloned human FP-receptor ( r = 0.9 ) , and rat uterus contraction ( r = 0.84 ) .
	manualset3
143611	12	409070	5	NULL	NULL	0	NULL	r = 0.77 - 0.86	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The cat iris contraction data were well correlated with other FP-receptor-mediated signal-transduction processes , including FP-receptor binding in bovine corpus luteum ( r = 0.86 ) , FP-receptor binding in human iris ( r = 0.61 ) , phosphoinositide ( PI ) hydrolysis in human ciliary muscle and trabecular meshwork cells ( r = 0.77 - 0.86 ) , PI turnover in rat and mouse cells ( r = 0.73 - 0.76 ) and via cloned human FP-receptor ( r = 0.9 ) , and rat uterus contraction ( r = 0.84 ) .
	manualset3
143612	13	409070	5	NULL	NULL	0	NULL	PI turnover	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cat iris contraction data were well correlated with other FP-receptor-mediated signal-transduction processes , including FP-receptor binding in bovine corpus luteum ( r = 0.86 ) , FP-receptor binding in human iris ( r = 0.61 ) , phosphoinositide ( PI ) hydrolysis in human ciliary muscle and trabecular meshwork cells ( r = 0.77 - 0.86 ) , PI turnover in rat and mouse cells ( r = 0.73 - 0.76 ) and via cloned human FP-receptor ( r = 0.9 ) , and rat uterus contraction ( r = 0.84 ) .
	manualset3
143613	14	409070	5	NULL	NULL	0	NULL	rat cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The cat iris contraction data were well correlated with other FP-receptor-mediated signal-transduction processes , including FP-receptor binding in bovine corpus luteum ( r = 0.86 ) , FP-receptor binding in human iris ( r = 0.61 ) , phosphoinositide ( PI ) hydrolysis in human ciliary muscle and trabecular meshwork cells ( r = 0.77 - 0.86 ) , PI turnover in rat and mouse cells ( r = 0.73 - 0.76 ) and via cloned human FP-receptor ( r = 0.9 ) , and rat uterus contraction ( r = 0.84 ) .
	manualset3
143614	15	409070	5	NULL	NULL	0	NULL	mouse cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The cat iris contraction data were well correlated with other FP-receptor-mediated signal-transduction processes , including FP-receptor binding in bovine corpus luteum ( r = 0.86 ) , FP-receptor binding in human iris ( r = 0.61 ) , phosphoinositide ( PI ) hydrolysis in human ciliary muscle and trabecular meshwork cells ( r = 0.77 - 0.86 ) , PI turnover in rat and mouse cells ( r = 0.73 - 0.76 ) and via cloned human FP-receptor ( r = 0.9 ) , and rat uterus contraction ( r = 0.84 ) .
	manualset3
143615	16	409070	5	NULL	NULL	0	NULL	r = 0.73 - 0.76	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The cat iris contraction data were well correlated with other FP-receptor-mediated signal-transduction processes , including FP-receptor binding in bovine corpus luteum ( r = 0.86 ) , FP-receptor binding in human iris ( r = 0.61 ) , phosphoinositide ( PI ) hydrolysis in human ciliary muscle and trabecular meshwork cells ( r = 0.77 - 0.86 ) , PI turnover in rat and mouse cells ( r = 0.73 - 0.76 ) and via cloned human FP-receptor ( r = 0.9 ) , and rat uterus contraction ( r = 0.84 ) .
	manualset3
143616	17	409070	5	NULL	NULL	0	NULL	cloned human FP-receptor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The cat iris contraction data were well correlated with other FP-receptor-mediated signal-transduction processes , including FP-receptor binding in bovine corpus luteum ( r = 0.86 ) , FP-receptor binding in human iris ( r = 0.61 ) , phosphoinositide ( PI ) hydrolysis in human ciliary muscle and trabecular meshwork cells ( r = 0.77 - 0.86 ) , PI turnover in rat and mouse cells ( r = 0.73 - 0.76 ) and via cloned human FP-receptor ( r = 0.9 ) , and rat uterus contraction ( r = 0.84 ) .
	manualset3
143617	18	409070	5	NULL	NULL	0	NULL	 r = 0.9	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The cat iris contraction data were well correlated with other FP-receptor-mediated signal-transduction processes , including FP-receptor binding in bovine corpus luteum ( r = 0.86 ) , FP-receptor binding in human iris ( r = 0.61 ) , phosphoinositide ( PI ) hydrolysis in human ciliary muscle and trabecular meshwork cells ( r = 0.77 - 0.86 ) , PI turnover in rat and mouse cells ( r = 0.73 - 0.76 ) and via cloned human FP-receptor ( r = 0.9 ) , and rat uterus contraction ( r = 0.84 ) .
	manualset3
143618	19	409070	5	NULL	NULL	0	NULL	rat uterus contraction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cat iris contraction data were well correlated with other FP-receptor-mediated signal-transduction processes , including FP-receptor binding in bovine corpus luteum ( r = 0.86 ) , FP-receptor binding in human iris ( r = 0.61 ) , phosphoinositide ( PI ) hydrolysis in human ciliary muscle and trabecular meshwork cells ( r = 0.77 - 0.86 ) , PI turnover in rat and mouse cells ( r = 0.73 - 0.76 ) and via cloned human FP-receptor ( r = 0.9 ) , and rat uterus contraction ( r = 0.84 ) .
	manualset3
143619	20	409070	5	NULL	NULL	0	NULL	r = 0.84	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The cat iris contraction data were well correlated with other FP-receptor-mediated signal-transduction processes , including FP-receptor binding in bovine corpus luteum ( r = 0.86 ) , FP-receptor binding in human iris ( r = 0.61 ) , phosphoinositide ( PI ) hydrolysis in human ciliary muscle and trabecular meshwork cells ( r = 0.77 - 0.86 ) , PI turnover in rat and mouse cells ( r = 0.73 - 0.76 ) and via cloned human FP-receptor ( r = 0.9 ) , and rat uterus contraction ( r = 0.84 ) .
	manualset3
143620	1	409071	5	NULL	NULL	0	NULL	catabolic action 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The catabolic action of glucagon in rat liver .
	manualset3
143621	2	409071	5	NULL	NULL	0	NULL	glucagon 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The catabolic action of glucagon in rat liver .
	manualset3
143622	3	409071	5	NULL	NULL	0	NULL	rat liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The catabolic action of glucagon in rat liver .
	manualset3
143623	1	409072	5	NULL	NULL	NULL	NULL	catalytic substitution reaction	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The catalytic substitution reaction proceeds with high regio - and stereoselectivity .
	manualset3
143624	2	409072	5	NULL	NULL	0	NULL	regio - and stereoselectivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The catalytic substitution reaction proceeds with high regio - and stereoselectivity .
	manualset3
143625	1	409073	5	NULL	NULL	0	NULL	cation retention 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cation retention of organoclays was dominated by the extent of hydrophobic interactions affected by the local distribution and arrangement of surfactants .
	manualset3
143626	2	409073	5	NULL	NULL	0	NULL	organoclays 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The cation retention of organoclays was dominated by the extent of hydrophobic interactions affected by the local distribution and arrangement of surfactants .
	manualset3
143627	3	409073	5	NULL	NULL	0	NULL	hydrophobic interactions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cation retention of organoclays was dominated by the extent of hydrophobic interactions affected by the local distribution and arrangement of surfactants .
	manualset3
143628	4	409073	5	NULL	NULL	0	NULL	local distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cation retention of organoclays was dominated by the extent of hydrophobic interactions affected by the local distribution and arrangement of surfactants .
	manualset3
143629	5	409073	5	NULL	NULL	0	NULL	arrangement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cation retention of organoclays was dominated by the extent of hydrophobic interactions affected by the local distribution and arrangement of surfactants .
	manualset3
143630	6	409073	5	NULL	NULL	0	NULL	surfactants 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The cation retention of organoclays was dominated by the extent of hydrophobic interactions affected by the local distribution and arrangement of surfactants .
	manualset3
143631	1	409074	5	NULL	NULL	0	NULL	causal common germ	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The causal common germ has been placed in a proeminent position in 18 cases ( 16.7 % ) including 14 cases of gram-positive germs .
	manualset3
143632	2	409074	5	NULL	NULL	0	NULL	proeminent position	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The causal common germ has been placed in a proeminent position in 18 cases ( 16.7 % ) including 14 cases of gram-positive germs .
	manualset3
143633	3	409074	5	NULL	NULL	0	NULL	18 cases ( 16.7 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The causal common germ has been placed in a proeminent position in 18 cases ( 16.7 % ) including 14 cases of gram-positive germs .
	manualset3
143634	4	409074	5	NULL	NULL	0	NULL	14 cases 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The causal common germ has been placed in a proeminent position in 18 cases ( 16.7 % ) including 14 cases of gram-positive germs .
	manualset3
143635	5	409074	5	NULL	NULL	0	NULL	gram-positive germs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The causal common germ has been placed in a proeminent position in 18 cases ( 16.7 % ) including 14 cases of gram-positive germs .
	manualset3
143636	1	409075	5	NULL	NULL	0	NULL	cause 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cause of death entered on the death certificates of 193 patients originally diagnosed as having cancer of the breast was compared with information obtained from clinical records , cancer registry records , and necropsy findings to determine the accuracy of death certification and the proportion of patients who , though dying from another cause , still had overt signs of cancer of the breast .
	manualset3
143637	2	409075	5	NULL	NULL	0	NULL	death 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cause of death entered on the death certificates of 193 patients originally diagnosed as having cancer of the breast was compared with information obtained from clinical records , cancer registry records , and necropsy findings to determine the accuracy of death certification and the proportion of patients who , though dying from another cause , still had overt signs of cancer of the breast .
	manualset3
143638	3	409075	5	NULL	NULL	0	NULL	death certificates 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The cause of death entered on the death certificates of 193 patients originally diagnosed as having cancer of the breast was compared with information obtained from clinical records , cancer registry records , and necropsy findings to determine the accuracy of death certification and the proportion of patients who , though dying from another cause , still had overt signs of cancer of the breast .
	manualset3
143639	4	409075	5	NULL	NULL	0	NULL	 193 patients	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The cause of death entered on the death certificates of 193 patients originally diagnosed as having cancer of the breast was compared with information obtained from clinical records , cancer registry records , and necropsy findings to determine the accuracy of death certification and the proportion of patients who , though dying from another cause , still had overt signs of cancer of the breast .
	manualset3
143640	5	409075	5	NULL	NULL	0	NULL	cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The cause of death entered on the death certificates of 193 patients originally diagnosed as having cancer of the breast was compared with information obtained from clinical records , cancer registry records , and necropsy findings to determine the accuracy of death certification and the proportion of patients who , though dying from another cause , still had overt signs of cancer of the breast .
	manualset3
143641	6	409075	5	NULL	NULL	0	NULL	breast 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The cause of death entered on the death certificates of 193 patients originally diagnosed as having cancer of the breast was compared with information obtained from clinical records , cancer registry records , and necropsy findings to determine the accuracy of death certification and the proportion of patients who , though dying from another cause , still had overt signs of cancer of the breast .
	manualset3
143642	7	409075	5	NULL	NULL	0	NULL	information 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cause of death entered on the death certificates of 193 patients originally diagnosed as having cancer of the breast was compared with information obtained from clinical records , cancer registry records , and necropsy findings to determine the accuracy of death certification and the proportion of patients who , though dying from another cause , still had overt signs of cancer of the breast .
	manualset3
143643	8	409075	5	NULL	NULL	0	NULL	clinical records	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The cause of death entered on the death certificates of 193 patients originally diagnosed as having cancer of the breast was compared with information obtained from clinical records , cancer registry records , and necropsy findings to determine the accuracy of death certification and the proportion of patients who , though dying from another cause , still had overt signs of cancer of the breast .
	manualset3
143644	9	409075	5	NULL	NULL	0	NULL	cancer registry records 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The cause of death entered on the death certificates of 193 patients originally diagnosed as having cancer of the breast was compared with information obtained from clinical records , cancer registry records , and necropsy findings to determine the accuracy of death certification and the proportion of patients who , though dying from another cause , still had overt signs of cancer of the breast .
	manualset3
143645	10	409075	5	NULL	NULL	0	NULL	necropsy findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cause of death entered on the death certificates of 193 patients originally diagnosed as having cancer of the breast was compared with information obtained from clinical records , cancer registry records , and necropsy findings to determine the accuracy of death certification and the proportion of patients who , though dying from another cause , still had overt signs of cancer of the breast .
	manualset3
143646	11	409075	5	NULL	NULL	0	NULL	accuracy 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cause of death entered on the death certificates of 193 patients originally diagnosed as having cancer of the breast was compared with information obtained from clinical records , cancer registry records , and necropsy findings to determine the accuracy of death certification and the proportion of patients who , though dying from another cause , still had overt signs of cancer of the breast .
	manualset3
143647	12	409075	5	NULL	NULL	0	NULL	death certification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cause of death entered on the death certificates of 193 patients originally diagnosed as having cancer of the breast was compared with information obtained from clinical records , cancer registry records , and necropsy findings to determine the accuracy of death certification and the proportion of patients who , though dying from another cause , still had overt signs of cancer of the breast .
	manualset3
143648	13	409075	5	NULL	NULL	0	NULL	proportion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cause of death entered on the death certificates of 193 patients originally diagnosed as having cancer of the breast was compared with information obtained from clinical records , cancer registry records , and necropsy findings to determine the accuracy of death certification and the proportion of patients who , though dying from another cause , still had overt signs of cancer of the breast .
	manualset3
143649	14	409075	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The cause of death entered on the death certificates of 193 patients originally diagnosed as having cancer of the breast was compared with information obtained from clinical records , cancer registry records , and necropsy findings to determine the accuracy of death certification and the proportion of patients who , though dying from another cause , still had overt signs of cancer of the breast .
	manualset3
143650	15	409075	5	NULL	NULL	0	NULL	cause 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cause of death entered on the death certificates of 193 patients originally diagnosed as having cancer of the breast was compared with information obtained from clinical records , cancer registry records , and necropsy findings to determine the accuracy of death certification and the proportion of patients who , though dying from another cause , still had overt signs of cancer of the breast .
	manualset3
143651	16	409075	5	NULL	NULL	0	NULL	overt signs 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cause of death entered on the death certificates of 193 patients originally diagnosed as having cancer of the breast was compared with information obtained from clinical records , cancer registry records , and necropsy findings to determine the accuracy of death certification and the proportion of patients who , though dying from another cause , still had overt signs of cancer of the breast .
	manualset3
143652	17	409075	5	NULL	NULL	0	NULL	cancer 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cause of death entered on the death certificates of 193 patients originally diagnosed as having cancer of the breast was compared with information obtained from clinical records , cancer registry records , and necropsy findings to determine the accuracy of death certification and the proportion of patients who , though dying from another cause , still had overt signs of cancer of the breast .
	manualset3
143653	18	409075	5	NULL	NULL	0	NULL	breast 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The cause of death entered on the death certificates of 193 patients originally diagnosed as having cancer of the breast was compared with information obtained from clinical records , cancer registry records , and necropsy findings to determine the accuracy of death certification and the proportion of patients who , though dying from another cause , still had overt signs of cancer of the breast .
	manualset3
143654	1	409076	5	NULL	NULL	0	NULL	cause 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cause of glucocorticoid resistance was GR negativity in these subclones .
	manualset3
143655	2	409076	5	NULL	NULL	0	NULL	glucocorticoid resistance	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cause of glucocorticoid resistance was GR negativity in these subclones .
	manualset3
143656	3	409076	5	NULL	NULL	0	NULL	GR negativity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cause of glucocorticoid resistance was GR negativity in these subclones .
	manualset3
143657	4	409076	5	NULL	NULL	0	NULL	subclones 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The cause of glucocorticoid resistance was GR negativity in these subclones .
	manualset3
143658	1	409077	5	NULL	NULL	0	NULL	cause 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cause of the dysphagia is often complex and related to a number of factors that are discussed .
	manualset3
143659	2	409077	5	NULL	NULL	0	NULL	dysphagia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cause of the dysphagia is often complex and related to a number of factors that are discussed .
	manualset3
143660	3	409077	5	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cause of the dysphagia is often complex and related to a number of factors that are discussed .
	manualset3
143661	4	409077	5	NULL	NULL	0	NULL	factors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cause of the dysphagia is often complex and related to a number of factors that are discussed .
	manualset3
143662	1	409078	5	NULL	NULL	0	NULL	cause 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cause which can determine it is not yet cleared up , although the Authors think the greatest responsibility for this can be ascribed to rejection .
	manualset3
143663	2	409078	5	NULL	NULL	0	NULL	Authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The cause which can determine it is not yet cleared up , although the Authors think the greatest responsibility for this can be ascribed to rejection .
	manualset3
143664	3	409078	5	NULL	NULL	0	NULL	responsibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cause which can determine it is not yet cleared up , although the Authors think the greatest responsibility for this can be ascribed to rejection .
	manualset3
143665	4	409078	5	NULL	NULL	0	NULL	rejection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cause which can determine it is not yet cleared up , although the Authors think the greatest responsibility for this can be ascribed to rejection .
	manualset3
143666	1	409079	5	NULL	NULL	0	NULL	causes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The causes of late mortality in ileostomists .
	manualset3
143667	2	409079	5	NULL	NULL	0	NULL	late mortality 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The causes of late mortality in ileostomists .
	manualset3
143668	3	409079	5	NULL	NULL	0	NULL	ileostomists 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The causes of late mortality in ileostomists .
	manualset3
143669	1	409080	5	NULL	NULL	0	NULL	causes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The causes of many renal diseases are not known but one must suspect immune-mediated damage in some .
	manualset3
143670	2	409080	5	NULL	NULL	0	NULL	renal diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The causes of many renal diseases are not known but one must suspect immune-mediated damage in some .
	manualset3
143671	3	409080	5	NULL	NULL	0	NULL	one 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The causes of many renal diseases are not known but one must suspect immune-mediated damage in some .
	manualset3
143672	4	409080	5	NULL	NULL	0	NULL	immune-mediated damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The causes of many renal diseases are not known but one must suspect immune-mediated damage in some .
	manualset3
143673	1	409081	5	NULL	NULL	0	NULL	causes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The causes of reoperation were recurrent spinal stenosis ( n = 3 ) , recurrent disc herniation ( n = 2 ) , post-laminectomy spondylolisthesis ( n = 1 ) , and delayed deep wound infection ( n = 1 ) .
	manualset3
143674	2	409081	5	NULL	NULL	0	NULL	reoperation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The causes of reoperation were recurrent spinal stenosis ( n = 3 ) , recurrent disc herniation ( n = 2 ) , post-laminectomy spondylolisthesis ( n = 1 ) , and delayed deep wound infection ( n = 1 ) .
	manualset3
143675	3	409081	5	NULL	NULL	0	NULL	recurrent spinal stenosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The causes of reoperation were recurrent spinal stenosis ( n = 3 ) , recurrent disc herniation ( n = 2 ) , post-laminectomy spondylolisthesis ( n = 1 ) , and delayed deep wound infection ( n = 1 ) .
	manualset3
143676	4	409081	5	NULL	NULL	0	NULL	 n = 3	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The causes of reoperation were recurrent spinal stenosis ( n = 3 ) , recurrent disc herniation ( n = 2 ) , post-laminectomy spondylolisthesis ( n = 1 ) , and delayed deep wound infection ( n = 1 ) .
	manualset3
143677	5	409081	5	NULL	NULL	0	NULL	recurrent disc herniation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The causes of reoperation were recurrent spinal stenosis ( n = 3 ) , recurrent disc herniation ( n = 2 ) , post-laminectomy spondylolisthesis ( n = 1 ) , and delayed deep wound infection ( n = 1 ) .
	manualset3
143678	6	409081	5	NULL	NULL	0	NULL	n = 2 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The causes of reoperation were recurrent spinal stenosis ( n = 3 ) , recurrent disc herniation ( n = 2 ) , post-laminectomy spondylolisthesis ( n = 1 ) , and delayed deep wound infection ( n = 1 ) .
	manualset3
143679	7	409081	5	NULL	NULL	0	NULL	post-laminectomy spondylolisthesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The causes of reoperation were recurrent spinal stenosis ( n = 3 ) , recurrent disc herniation ( n = 2 ) , post-laminectomy spondylolisthesis ( n = 1 ) , and delayed deep wound infection ( n = 1 ) .
	manualset3
143680	8	409081	5	NULL	NULL	0	NULL	n = 1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The causes of reoperation were recurrent spinal stenosis ( n = 3 ) , recurrent disc herniation ( n = 2 ) , post-laminectomy spondylolisthesis ( n = 1 ) , and delayed deep wound infection ( n = 1 ) .
	manualset3
143681	9	409081	5	NULL	NULL	0	NULL	delayed deep wound infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The causes of reoperation were recurrent spinal stenosis ( n = 3 ) , recurrent disc herniation ( n = 2 ) , post-laminectomy spondylolisthesis ( n = 1 ) , and delayed deep wound infection ( n = 1 ) .
	manualset3
143682	10	409081	5	NULL	NULL	0	NULL	n = 1 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The causes of reoperation were recurrent spinal stenosis ( n = 3 ) , recurrent disc herniation ( n = 2 ) , post-laminectomy spondylolisthesis ( n = 1 ) , and delayed deep wound infection ( n = 1 ) .
	manualset3
143683	1	409082	5	NULL	NULL	0	NULL	cell cycle 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cell cycle and beyond : an interview with Paul Nurse .
	manualset3
143684	2	409082	5	NULL	NULL	0	NULL	interview 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cell cycle and beyond : an interview with Paul Nurse .
	manualset3
143685	3	409082	5	NULL	NULL	0	NULL	Paul Nurse	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The cell cycle and beyond : an interview with Paul Nurse .
	manualset3
143686	1	409083	5	NULL	NULL	0	NULL	 cell cycle perturbation effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cell cycle perturbation effect is suggested to be one of the critical factors for the detection of the clastogenic potential of IQ .
	manualset3
143687	2	409083	5	NULL	NULL	0	NULL	one 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The cell cycle perturbation effect is suggested to be one of the critical factors for the detection of the clastogenic potential of IQ .
	manualset3
143688	3	409083	5	NULL	NULL	0	NULL	critical factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cell cycle perturbation effect is suggested to be one of the critical factors for the detection of the clastogenic potential of IQ .
	manualset3
143689	4	409083	5	NULL	NULL	0	NULL	detection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cell cycle perturbation effect is suggested to be one of the critical factors for the detection of the clastogenic potential of IQ .
	manualset3
143690	5	409083	5	NULL	NULL	NULL	NULL	clastogenic potential	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The cell cycle perturbation effect is suggested to be one of the critical factors for the detection of the clastogenic potential of IQ .
	manualset3
143691	6	409083	5	NULL	NULL	0	NULL	IQ 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The cell cycle perturbation effect is suggested to be one of the critical factors for the detection of the clastogenic potential of IQ .
	manualset3
143692	1	409084	5	NULL	NULL	0	NULL	 cell death patterns	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cell death patterns appear to be pathogenically correlated with subsequently observed malformations including exencephaly ( anencephaly ) , arhinencephaly , pituitary dysplasia , bilateral or unilateral cleft lip , maxillary hypoplasia , and median facial deficiencies and clefts .
	manualset3
143693	2	409084	5	NULL	NULL	0	NULL	malformations 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cell death patterns appear to be pathogenically correlated with subsequently observed malformations including exencephaly ( anencephaly ) , arhinencephaly , pituitary dysplasia , bilateral or unilateral cleft lip , maxillary hypoplasia , and median facial deficiencies and clefts .
	manualset3
143694	3	409084	5	NULL	NULL	NULL	NULL	exencephaly ( anencephaly ) 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The cell death patterns appear to be pathogenically correlated with subsequently observed malformations including exencephaly ( anencephaly ) , arhinencephaly , pituitary dysplasia , bilateral or unilateral cleft lip , maxillary hypoplasia , and median facial deficiencies and clefts .
	manualset3
143695	4	409084	5	NULL	NULL	0	NULL	arhinencephaly 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The cell death patterns appear to be pathogenically correlated with subsequently observed malformations including exencephaly ( anencephaly ) , arhinencephaly , pituitary dysplasia , bilateral or unilateral cleft lip , maxillary hypoplasia , and median facial deficiencies and clefts .
	manualset3
143696	5	409084	5	NULL	NULL	0	NULL	pituitary dysplasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cell death patterns appear to be pathogenically correlated with subsequently observed malformations including exencephaly ( anencephaly ) , arhinencephaly , pituitary dysplasia , bilateral or unilateral cleft lip , maxillary hypoplasia , and median facial deficiencies and clefts .
	manualset3
143697	6	409084	5	NULL	NULL	0	NULL	bilateral or unilateral cleft lip	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cell death patterns appear to be pathogenically correlated with subsequently observed malformations including exencephaly ( anencephaly ) , arhinencephaly , pituitary dysplasia , bilateral or unilateral cleft lip , maxillary hypoplasia , and median facial deficiencies and clefts .
	manualset3
143698	7	409084	5	NULL	NULL	0	NULL	maxillary hypoplasia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cell death patterns appear to be pathogenically correlated with subsequently observed malformations including exencephaly ( anencephaly ) , arhinencephaly , pituitary dysplasia , bilateral or unilateral cleft lip , maxillary hypoplasia , and median facial deficiencies and clefts .
	manualset3
143699	8	409084	5	NULL	NULL	0	NULL	median facial deficiencies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cell death patterns appear to be pathogenically correlated with subsequently observed malformations including exencephaly ( anencephaly ) , arhinencephaly , pituitary dysplasia , bilateral or unilateral cleft lip , maxillary hypoplasia , and median facial deficiencies and clefts .
	manualset3
143700	9	409084	5	NULL	NULL	0	NULL	clefts 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cell death patterns appear to be pathogenically correlated with subsequently observed malformations including exencephaly ( anencephaly ) , arhinencephaly , pituitary dysplasia , bilateral or unilateral cleft lip , maxillary hypoplasia , and median facial deficiencies and clefts .
	manualset3
143701	1	409085	5	NULL	NULL	0	NULL	cell 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The cell displays all the essential hepatocyte function , and may replace the mature hepatocyte for regenerative medicine of the liver .
	manualset3
143702	2	409085	5	NULL	NULL	0	NULL	hepatocyte function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cell displays all the essential hepatocyte function , and may replace the mature hepatocyte for regenerative medicine of the liver .
	manualset3
143703	3	409085	5	NULL	NULL	0	NULL	mature hepatocyte 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The cell displays all the essential hepatocyte function , and may replace the mature hepatocyte for regenerative medicine of the liver .
	manualset3
143704	4	409085	5	NULL	NULL	0	NULL	regenerative medicine	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The cell displays all the essential hepatocyte function , and may replace the mature hepatocyte for regenerative medicine of the liver .
	manualset3
143705	5	409085	5	NULL	NULL	0	NULL	liver 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The cell displays all the essential hepatocyte function , and may replace the mature hepatocyte for regenerative medicine of the liver .
	manualset3
143706	1	409086	5	NULL	NULL	0	NULL	cell surface	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The cell surface is partly covered by basement membrane .
	manualset3
143707	2	409086	5	NULL	NULL	NULL	NULL	basement membrane	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The cell surface is partly covered by basement membrane .
	manualset3
143708	1	409087	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The cells also contained large hexagonal bodies , rod-shaped fibrillar elements , and polyphosphate granules .
	manualset3
143709	2	409087	5	NULL	NULL	0	NULL	large hexagonal bodies	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The cells also contained large hexagonal bodies , rod-shaped fibrillar elements , and polyphosphate granules .
	manualset3
143710	3	409087	5	NULL	NULL	0	NULL	rod-shaped fibrillar elements	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The cells also contained large hexagonal bodies , rod-shaped fibrillar elements , and polyphosphate granules .
	manualset3
143711	4	409087	5	NULL	NULL	0	NULL	polyphosphate granules	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The cells also contained large hexagonal bodies , rod-shaped fibrillar elements , and polyphosphate granules .
	manualset3
143712	1	409088	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The cells were eluted from the beads and lysed by heating ; the eluate was then assayed by real-time PCR , using primers and probe specifically targeting the eaeA gene of E. coli O157 : H7 .
	manualset3
143713	2	409088	5	NULL	NULL	0	NULL	beads 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The cells were eluted from the beads and lysed by heating ; the eluate was then assayed by real-time PCR , using primers and probe specifically targeting the eaeA gene of E. coli O157 : H7 .
	manualset3
143714	3	409088	5	NULL	NULL	0	NULL	heating 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cells were eluted from the beads and lysed by heating ; the eluate was then assayed by real-time PCR , using primers and probe specifically targeting the eaeA gene of E. coli O157 : H7 .
	manualset3
143715	4	409088	5	NULL	NULL	0	NULL	eluate 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The cells were eluted from the beads and lysed by heating ; the eluate was then assayed by real-time PCR , using primers and probe specifically targeting the eaeA gene of E. coli O157 : H7 .
	manualset3
143716	5	409088	5	NULL	NULL	0	NULL	real-time PCR 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The cells were eluted from the beads and lysed by heating ; the eluate was then assayed by real-time PCR , using primers and probe specifically targeting the eaeA gene of E. coli O157 : H7 .
	manualset3
143717	6	409088	5	NULL	NULL	0	NULL	primers 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The cells were eluted from the beads and lysed by heating ; the eluate was then assayed by real-time PCR , using primers and probe specifically targeting the eaeA gene of E. coli O157 : H7 .
	manualset3
143718	7	409088	5	NULL	NULL	0	NULL	probe 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The cells were eluted from the beads and lysed by heating ; the eluate was then assayed by real-time PCR , using primers and probe specifically targeting the eaeA gene of E. coli O157 : H7 .
	manualset3
143719	8	409088	5	NULL	NULL	0	NULL	eaeA gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The cells were eluted from the beads and lysed by heating ; the eluate was then assayed by real-time PCR , using primers and probe specifically targeting the eaeA gene of E. coli O157 : H7 .
	manualset3
143720	9	409088	5	NULL	NULL	0	NULL	E. coli O157 : H7	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The cells were eluted from the beads and lysed by heating ; the eluate was then assayed by real-time PCR , using primers and probe specifically targeting the eaeA gene of E. coli O157 : H7 .
	manualset3
143721	1	409089	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The cells were grown directly on slides in order to minimize damage to them during manipulation and to avoid trypsin treatment .
	manualset3
143722	2	409089	5	NULL	NULL	0	NULL	slides 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The cells were grown directly on slides in order to minimize damage to them during manipulation and to avoid trypsin treatment .
	manualset3
143723	3	409089	5	NULL	NULL	0	NULL	damage 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cells were grown directly on slides in order to minimize damage to them during manipulation and to avoid trypsin treatment .
	manualset3
143724	4	409089	5	NULL	NULL	NULL	NULL	manipulation 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The cells were grown directly on slides in order to minimize damage to them during manipulation and to avoid trypsin treatment .
	manualset3
143725	5	409089	5	NULL	NULL	0	NULL	trypsin treatment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cells were grown directly on slides in order to minimize damage to them during manipulation and to avoid trypsin treatment .
	manualset3
143726	1	409090	5	NULL	NULL	0	NULL	cellular clock 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cellular clock is based on a network of core clock genes , which drive the circadian expression of non-clock genes involved in many cellular processes .
	manualset3
143727	2	409090	5	NULL	NULL	0	NULL	network 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cellular clock is based on a network of core clock genes , which drive the circadian expression of non-clock genes involved in many cellular processes .
	manualset3
143728	3	409090	5	NULL	NULL	0	NULL	core clock genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The cellular clock is based on a network of core clock genes , which drive the circadian expression of non-clock genes involved in many cellular processes .
	manualset3
143729	4	409090	5	NULL	NULL	0	NULL	circadian expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cellular clock is based on a network of core clock genes , which drive the circadian expression of non-clock genes involved in many cellular processes .
	manualset3
143730	5	409090	5	NULL	NULL	0	NULL	non-clock genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The cellular clock is based on a network of core clock genes , which drive the circadian expression of non-clock genes involved in many cellular processes .
	manualset3
143731	6	409090	5	NULL	NULL	0	NULL	cellular processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cellular clock is based on a network of core clock genes , which drive the circadian expression of non-clock genes involved in many cellular processes .
	manualset3
143732	1	409091	5	NULL	NULL	0	NULL	series 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of pharmacokinetic and metabolic profile studies on epsilon - polylysine have been conducted in rats in order to provide a better understanding of the reason for its lack of toxicological effects in subchronic and chronic feeding bioassays using relatively high concentrations in the diet up to 50000 ppm .
	manualset3
143733	2	409091	5	NULL	NULL	0	NULL	pharmacokinetic profile studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of pharmacokinetic and metabolic profile studies on epsilon - polylysine have been conducted in rats in order to provide a better understanding of the reason for its lack of toxicological effects in subchronic and chronic feeding bioassays using relatively high concentrations in the diet up to 50000 ppm .
	manualset3
143734	3	409091	5	NULL	NULL	0	NULL	metabolic profile studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of pharmacokinetic and metabolic profile studies on epsilon - polylysine have been conducted in rats in order to provide a better understanding of the reason for its lack of toxicological effects in subchronic and chronic feeding bioassays using relatively high concentrations in the diet up to 50000 ppm .
	manualset3
143735	4	409091	5	NULL	NULL	0	NULL	epsilon - polylysine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of pharmacokinetic and metabolic profile studies on epsilon - polylysine have been conducted in rats in order to provide a better understanding of the reason for its lack of toxicological effects in subchronic and chronic feeding bioassays using relatively high concentrations in the diet up to 50000 ppm .
	manualset3
143736	5	409091	5	NULL	NULL	0	NULL	rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of pharmacokinetic and metabolic profile studies on epsilon - polylysine have been conducted in rats in order to provide a better understanding of the reason for its lack of toxicological effects in subchronic and chronic feeding bioassays using relatively high concentrations in the diet up to 50000 ppm .
	manualset3
143737	6	409091	5	NULL	NULL	0	NULL	understanding 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of pharmacokinetic and metabolic profile studies on epsilon - polylysine have been conducted in rats in order to provide a better understanding of the reason for its lack of toxicological effects in subchronic and chronic feeding bioassays using relatively high concentrations in the diet up to 50000 ppm .
	manualset3
143738	7	409091	5	NULL	NULL	0	NULL	reason 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of pharmacokinetic and metabolic profile studies on epsilon - polylysine have been conducted in rats in order to provide a better understanding of the reason for its lack of toxicological effects in subchronic and chronic feeding bioassays using relatively high concentrations in the diet up to 50000 ppm .
	manualset3
143739	8	409091	5	NULL	NULL	0	NULL	toxicological effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of pharmacokinetic and metabolic profile studies on epsilon - polylysine have been conducted in rats in order to provide a better understanding of the reason for its lack of toxicological effects in subchronic and chronic feeding bioassays using relatively high concentrations in the diet up to 50000 ppm .
	manualset3
143740	9	409091	5	NULL	NULL	0	NULL	subchronic feeding bioassay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of pharmacokinetic and metabolic profile studies on epsilon - polylysine have been conducted in rats in order to provide a better understanding of the reason for its lack of toxicological effects in subchronic and chronic feeding bioassays using relatively high concentrations in the diet up to 50000 ppm .
	manualset3
143741	10	409091	5	NULL	NULL	0	NULL	chronic feeding bioassay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of pharmacokinetic and metabolic profile studies on epsilon - polylysine have been conducted in rats in order to provide a better understanding of the reason for its lack of toxicological effects in subchronic and chronic feeding bioassays using relatively high concentrations in the diet up to 50000 ppm .
	manualset3
143742	11	409091	5	NULL	NULL	0	NULL	concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of pharmacokinetic and metabolic profile studies on epsilon - polylysine have been conducted in rats in order to provide a better understanding of the reason for its lack of toxicological effects in subchronic and chronic feeding bioassays using relatively high concentrations in the diet up to 50000 ppm .
	manualset3
143743	12	409091	5	NULL	NULL	0	NULL	diet 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of pharmacokinetic and metabolic profile studies on epsilon - polylysine have been conducted in rats in order to provide a better understanding of the reason for its lack of toxicological effects in subchronic and chronic feeding bioassays using relatively high concentrations in the diet up to 50000 ppm .
	manualset3
143744	13	409091	5	NULL	NULL	0	NULL	50000 ppm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of pharmacokinetic and metabolic profile studies on epsilon - polylysine have been conducted in rats in order to provide a better understanding of the reason for its lack of toxicological effects in subchronic and chronic feeding bioassays using relatively high concentrations in the diet up to 50000 ppm .
	manualset3
143745	1	409092	5	NULL	NULL	0	NULL	cellular mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cellular mechanism of the hyperpolarization-induced vasodilatation remains unclear , and this should be clarified in the future for further understanding of the EDHF-induced vasodilatation .
	manualset3
143746	2	409092	5	NULL	NULL	0	NULL	hyperpolarization-induced vasodilatation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cellular mechanism of the hyperpolarization-induced vasodilatation remains unclear , and this should be clarified in the future for further understanding of the EDHF-induced vasodilatation .
	manualset3
143747	3	409092	5	NULL	NULL	0	NULL	future 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The cellular mechanism of the hyperpolarization-induced vasodilatation remains unclear , and this should be clarified in the future for further understanding of the EDHF-induced vasodilatation .
	manualset3
143748	4	409092	5	NULL	NULL	0	NULL	understanding 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cellular mechanism of the hyperpolarization-induced vasodilatation remains unclear , and this should be clarified in the future for further understanding of the EDHF-induced vasodilatation .
	manualset3
143749	5	409092	5	NULL	NULL	0	NULL	EDHF-induced vasodilatation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cellular mechanism of the hyperpolarization-induced vasodilatation remains unclear , and this should be clarified in the future for further understanding of the EDHF-induced vasodilatation .
	manualset3
143750	1	409093	5	NULL	NULL	0	NULL	cellular morphology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cellular morphology of all transfected GH ( 4 ) C ( 1 ) cell clones showed moderate differences to untransfected GH ( 4 ) C ( 1 ) cells .
	manualset3
143751	2	409093	5	NULL	NULL	0	NULL	transfected GH ( 4 ) C ( 1 ) cell clones	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The cellular morphology of all transfected GH ( 4 ) C ( 1 ) cell clones showed moderate differences to untransfected GH ( 4 ) C ( 1 ) cells .
	manualset3
143752	3	409093	5	NULL	NULL	0	NULL	differences 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cellular morphology of all transfected GH ( 4 ) C ( 1 ) cell clones showed moderate differences to untransfected GH ( 4 ) C ( 1 ) cells .
	manualset3
143753	4	409093	5	NULL	NULL	0	NULL	untransfected GH ( 4 ) C ( 1 ) cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The cellular morphology of all transfected GH ( 4 ) C ( 1 ) cell clones showed moderate differences to untransfected GH ( 4 ) C ( 1 ) cells .
	manualset3
143754	1	409094	5	NULL	NULL	0	NULL	centennial year	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The centennial year : the development of important ideas during the last 100 years .
	manualset3
143755	2	409094	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The centennial year : the development of important ideas during the last 100 years .
	manualset3
143756	3	409094	5	NULL	NULL	0	NULL	ideas 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The centennial year : the development of important ideas during the last 100 years .
	manualset3
143757	4	409094	5	NULL	NULL	0	NULL	 100 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The centennial year : the development of important ideas during the last 100 years .
	manualset3
143758	1	409095	5	NULL	NULL	0	NULL	 central globular H1 domain 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The central globular H1 domain asymmetrically interacts with DNA at the exit or entry end of the nucleosomal core DNA , and the C-terminal domain has a major impact on the linker DNA conformation and chromatin condensation .
	manualset3
143759	2	409095	5	NULL	NULL	0	NULL	DNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The central globular H1 domain asymmetrically interacts with DNA at the exit or entry end of the nucleosomal core DNA , and the C-terminal domain has a major impact on the linker DNA conformation and chromatin condensation .
	manualset3
143760	3	409095	5	NULL	NULL	0	NULL	exit or entry end of the nucleosomal core DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The central globular H1 domain asymmetrically interacts with DNA at the exit or entry end of the nucleosomal core DNA , and the C-terminal domain has a major impact on the linker DNA conformation and chromatin condensation .
	manualset3
143761	4	409095	5	NULL	NULL	0	NULL	C-terminal domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The central globular H1 domain asymmetrically interacts with DNA at the exit or entry end of the nucleosomal core DNA , and the C-terminal domain has a major impact on the linker DNA conformation and chromatin condensation .
	manualset3
143762	5	409095	5	NULL	NULL	0	NULL	major impact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The central globular H1 domain asymmetrically interacts with DNA at the exit or entry end of the nucleosomal core DNA , and the C-terminal domain has a major impact on the linker DNA conformation and chromatin condensation .
	manualset3
143763	6	409095	5	NULL	NULL	NULL	NULL	linker DNA conformation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The central globular H1 domain asymmetrically interacts with DNA at the exit or entry end of the nucleosomal core DNA , and the C-terminal domain has a major impact on the linker DNA conformation and chromatin condensation .
	manualset3
143764	7	409095	5	NULL	NULL	0	NULL	chromatin condensation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The central globular H1 domain asymmetrically interacts with DNA at the exit or entry end of the nucleosomal core DNA , and the C-terminal domain has a major impact on the linker DNA conformation and chromatin condensation .
	manualset3
143765	1	409096	5	NULL	NULL	0	NULL	central position	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The central position of LH-RH and the factors influencing its secretion , the negative feedback between the testicular hormones including inhibin and the hypophyseal gonadotropins as well as the periodic changes superimposed to the basal secretion of the sexual hormones are explained .
	manualset3
143766	2	409096	5	NULL	NULL	0	NULL	LH-RH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The central position of LH-RH and the factors influencing its secretion , the negative feedback between the testicular hormones including inhibin and the hypophyseal gonadotropins as well as the periodic changes superimposed to the basal secretion of the sexual hormones are explained .
	manualset3
143767	3	409096	5	NULL	NULL	0	NULL	factors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The central position of LH-RH and the factors influencing its secretion , the negative feedback between the testicular hormones including inhibin and the hypophyseal gonadotropins as well as the periodic changes superimposed to the basal secretion of the sexual hormones are explained .
	manualset3
143768	4	409096	5	NULL	NULL	0	NULL	secretion 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The central position of LH-RH and the factors influencing its secretion , the negative feedback between the testicular hormones including inhibin and the hypophyseal gonadotropins as well as the periodic changes superimposed to the basal secretion of the sexual hormones are explained .
	manualset3
143769	5	409096	5	NULL	NULL	0	NULL	negative feedback	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The central position of LH-RH and the factors influencing its secretion , the negative feedback between the testicular hormones including inhibin and the hypophyseal gonadotropins as well as the periodic changes superimposed to the basal secretion of the sexual hormones are explained .
	manualset3
143770	6	409096	5	NULL	NULL	NULL	NULL	testicular hormones	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The central position of LH-RH and the factors influencing its secretion , the negative feedback between the testicular hormones including inhibin and the hypophyseal gonadotropins as well as the periodic changes superimposed to the basal secretion of the sexual hormones are explained .
	manualset3
143771	7	409096	5	NULL	NULL	0	NULL	inhibin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The central position of LH-RH and the factors influencing its secretion , the negative feedback between the testicular hormones including inhibin and the hypophyseal gonadotropins as well as the periodic changes superimposed to the basal secretion of the sexual hormones are explained .
	manualset3
143772	8	409096	5	NULL	NULL	0	NULL	hypophyseal gonadotropins 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The central position of LH-RH and the factors influencing its secretion , the negative feedback between the testicular hormones including inhibin and the hypophyseal gonadotropins as well as the periodic changes superimposed to the basal secretion of the sexual hormones are explained .
	manualset3
143773	9	409096	5	NULL	NULL	0	NULL	periodic changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The central position of LH-RH and the factors influencing its secretion , the negative feedback between the testicular hormones including inhibin and the hypophyseal gonadotropins as well as the periodic changes superimposed to the basal secretion of the sexual hormones are explained .
	manualset3
143774	10	409096	5	NULL	NULL	0	NULL	basal secretion 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The central position of LH-RH and the factors influencing its secretion , the negative feedback between the testicular hormones including inhibin and the hypophyseal gonadotropins as well as the periodic changes superimposed to the basal secretion of the sexual hormones are explained .
	manualset3
143775	11	409096	5	NULL	NULL	0	NULL	sexual hormones	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The central position of LH-RH and the factors influencing its secretion , the negative feedback between the testicular hormones including inhibin and the hypophyseal gonadotropins as well as the periodic changes superimposed to the basal secretion of the sexual hormones are explained .
	manualset3
143776	1	409097	5	NULL	NULL	0	NULL	cerebral circulatory effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cerebral circulatory effects of the intracarotid administration of 5-hydroxytryptamine were examined in anaesthetized baboons .
	manualset3
143777	2	409097	5	NULL	NULL	0	NULL	intracarotid administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The cerebral circulatory effects of the intracarotid administration of 5-hydroxytryptamine were examined in anaesthetized baboons .
	manualset3
143778	3	409097	5	NULL	NULL	0	NULL	5-hydroxytryptamine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The cerebral circulatory effects of the intracarotid administration of 5-hydroxytryptamine were examined in anaesthetized baboons .
	manualset3
143779	4	409097	5	NULL	NULL	0	NULL	anaesthetized baboons	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The cerebral circulatory effects of the intracarotid administration of 5-hydroxytryptamine were examined in anaesthetized baboons .
	manualset3
143780	1	409098	5	NULL	NULL	0	NULL	cerebrospinal fluid ( CSF )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The cerebrospinal fluid ( CSF ) was bloody and the CSF pressure was 220 mm H2O .
	manualset3
143781	2	409098	5	NULL	NULL	0	NULL	 CSF pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cerebrospinal fluid ( CSF ) was bloody and the CSF pressure was 220 mm H2O .
	manualset3
143782	3	409098	5	NULL	NULL	0	NULL	220 mm H2O	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The cerebrospinal fluid ( CSF ) was bloody and the CSF pressure was 220 mm H2O .
	manualset3
143783	1	409099	5	NULL	NULL	0	NULL	chains 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The chains are further connected through N-HO and O-HO hydrogen bonds between the complex mol-ecule and an uncoordinated benzene-1 , 3 - dicarboxylic acid mol-ecule , resulting in a two-dimensional supra-molecular network .
	manualset3
143784	2	409099	5	NULL	NULL	0	NULL	N-HO hydrogen bond	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The chains are further connected through N-HO and O-HO hydrogen bonds between the complex mol-ecule and an uncoordinated benzene-1 , 3 - dicarboxylic acid mol-ecule , resulting in a two-dimensional supra-molecular network .
	manualset3
143785	3	409099	5	NULL	NULL	0	NULL	O-HO hydrogen bond	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The chains are further connected through N-HO and O-HO hydrogen bonds between the complex mol-ecule and an uncoordinated benzene-1 , 3 - dicarboxylic acid mol-ecule , resulting in a two-dimensional supra-molecular network .
	manualset3
143786	4	409099	5	NULL	NULL	0	NULL	complex mol-ecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The chains are further connected through N-HO and O-HO hydrogen bonds between the complex mol-ecule and an uncoordinated benzene-1 , 3 - dicarboxylic acid mol-ecule , resulting in a two-dimensional supra-molecular network .
	manualset3
143787	5	409099	5	NULL	NULL	0	NULL	benzene-1 , 3 - dicarboxylic acid mol-ecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The chains are further connected through N-HO and O-HO hydrogen bonds between the complex mol-ecule and an uncoordinated benzene-1 , 3 - dicarboxylic acid mol-ecule , resulting in a two-dimensional supra-molecular network .
	manualset3
143788	6	409099	5	NULL	NULL	0	NULL	two-dimensional supra-molecular network	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The chains are further connected through N-HO and O-HO hydrogen bonds between the complex mol-ecule and an uncoordinated benzene-1 , 3 - dicarboxylic acid mol-ecule , resulting in a two-dimensional supra-molecular network .
	manualset3
143789	1	409100	5	NULL	NULL	0	NULL	server 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A server for genotyping of mumps virus is developed and made available at http : //bioinfo.net.in/muv/homepage.html .
	manualset3
143790	2	409100	5	NULL	NULL	0	NULL	genotyping 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A server for genotyping of mumps virus is developed and made available at http : //bioinfo.net.in/muv/homepage.html .
	manualset3
143791	3	409100	5	NULL	NULL	0	NULL	mumps virus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A server for genotyping of mumps virus is developed and made available at http : //bioinfo.net.in/muv/homepage.html .
	manualset3
143792	4	409100	5	NULL	NULL	NULL	NULL	http : //bioinfo.net.in/muv/homepage.html	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A server for genotyping of mumps virus is developed and made available at http : //bioinfo.net.in/muv/homepage.html .
	manualset3
143793	1	409101	5	NULL	NULL	0	NULL	challenge 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The challenge of cross-cultural assessment -- The Test of Ability To Explain for Zulu-speaking Children .
	manualset3
143794	2	409101	5	NULL	NULL	0	NULL	cross-cultural assessment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The challenge of cross-cultural assessment -- The Test of Ability To Explain for Zulu-speaking Children .
	manualset3
143795	3	409101	5	NULL	NULL	0	NULL	Test of Ability 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The challenge of cross-cultural assessment -- The Test of Ability To Explain for Zulu-speaking Children .
	manualset3
143796	4	409101	5	NULL	NULL	0	NULL	Explain 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The challenge of cross-cultural assessment -- The Test of Ability To Explain for Zulu-speaking Children .
	manualset3
143797	5	409101	5	NULL	NULL	0	NULL	Zulu-speaking Children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The challenge of cross-cultural assessment -- The Test of Ability To Explain for Zulu-speaking Children .
	manualset3
143798	1	409102	5	NULL	NULL	0	NULL	challenge 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The challenge to clinicians is to differentiate normal patterns of jaundice and hyperbilirubinemia from those that indicate an abnormality or place an infant at risk .
	manualset3
143799	2	409102	5	NULL	NULL	0	NULL	clinicians 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The challenge to clinicians is to differentiate normal patterns of jaundice and hyperbilirubinemia from those that indicate an abnormality or place an infant at risk .
	manualset3
143800	3	409102	5	NULL	NULL	0	NULL	normal patterns 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The challenge to clinicians is to differentiate normal patterns of jaundice and hyperbilirubinemia from those that indicate an abnormality or place an infant at risk .
	manualset3
143801	4	409102	5	NULL	NULL	0	NULL	jaundice 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The challenge to clinicians is to differentiate normal patterns of jaundice and hyperbilirubinemia from those that indicate an abnormality or place an infant at risk .
	manualset3
143802	5	409102	5	NULL	NULL	0	NULL	hyperbilirubinemia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The challenge to clinicians is to differentiate normal patterns of jaundice and hyperbilirubinemia from those that indicate an abnormality or place an infant at risk .
	manualset3
143803	6	409102	5	NULL	NULL	0	NULL	abnormality 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The challenge to clinicians is to differentiate normal patterns of jaundice and hyperbilirubinemia from those that indicate an abnormality or place an infant at risk .
	manualset3
143804	7	409102	5	NULL	NULL	0	NULL	infant 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The challenge to clinicians is to differentiate normal patterns of jaundice and hyperbilirubinemia from those that indicate an abnormality or place an infant at risk .
	manualset3
143805	8	409102	5	NULL	NULL	0	NULL	risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The challenge to clinicians is to differentiate normal patterns of jaundice and hyperbilirubinemia from those that indicate an abnormality or place an infant at risk .
	manualset3
143806	1	409103	5	NULL	NULL	0	NULL	challenges 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The challenges become even more daunting when there is possible hazmat exposure as well ; this means that adequate and rapid disposition of victims is even more critical in order to avoid contamination of hospitals systems or whole communities .
	manualset3
143807	2	409103	5	NULL	NULL	0	NULL	hazmat exposure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The challenges become even more daunting when there is possible hazmat exposure as well ; this means that adequate and rapid disposition of victims is even more critical in order to avoid contamination of hospitals systems or whole communities .
	manualset3
143808	3	409103	5	NULL	NULL	NULL	NULL	rapid disposition 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The challenges become even more daunting when there is possible hazmat exposure as well ; this means that adequate and rapid disposition of victims is even more critical in order to avoid contamination of hospitals systems or whole communities .
	manualset3
143809	4	409103	5	NULL	NULL	0	NULL	victims 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The challenges become even more daunting when there is possible hazmat exposure as well ; this means that adequate and rapid disposition of victims is even more critical in order to avoid contamination of hospitals systems or whole communities .
	manualset3
143810	5	409103	5	NULL	NULL	0	NULL	contamination 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The challenges become even more daunting when there is possible hazmat exposure as well ; this means that adequate and rapid disposition of victims is even more critical in order to avoid contamination of hospitals systems or whole communities .
	manualset3
143811	6	409103	5	NULL	NULL	0	NULL	hospitals systems	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The challenges become even more daunting when there is possible hazmat exposure as well ; this means that adequate and rapid disposition of victims is even more critical in order to avoid contamination of hospitals systems or whole communities .
	manualset3
143812	7	409103	5	NULL	NULL	0	NULL	whole communities	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The challenges become even more daunting when there is possible hazmat exposure as well ; this means that adequate and rapid disposition of victims is even more critical in order to avoid contamination of hospitals systems or whole communities .
	manualset3
143813	1	409104	5	NULL	NULL	0	NULL	challenges 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The challenges of prompt identification and resuscitation in children with acute fulminant myocarditis : case series and review of the literature .
	manualset3
143814	2	409104	5	NULL	NULL	0	NULL	prompt identification	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The challenges of prompt identification and resuscitation in children with acute fulminant myocarditis : case series and review of the literature .
	manualset3
143815	3	409104	5	NULL	NULL	0	NULL	resuscitation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The challenges of prompt identification and resuscitation in children with acute fulminant myocarditis : case series and review of the literature .
	manualset3
143816	4	409104	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The challenges of prompt identification and resuscitation in children with acute fulminant myocarditis : case series and review of the literature .
	manualset3
143817	5	409104	5	NULL	NULL	0	NULL	acute fulminant myocarditis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The challenges of prompt identification and resuscitation in children with acute fulminant myocarditis : case series and review of the literature .
	manualset3
143818	6	409104	5	NULL	NULL	0	NULL	 case series	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The challenges of prompt identification and resuscitation in children with acute fulminant myocarditis : case series and review of the literature .
	manualset3
143819	7	409104	5	NULL	NULL	0	NULL	review 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The challenges of prompt identification and resuscitation in children with acute fulminant myocarditis : case series and review of the literature .
	manualset3
143820	8	409104	5	NULL	NULL	0	NULL	literature 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The challenges of prompt identification and resuscitation in children with acute fulminant myocarditis : case series and review of the literature .
	manualset3
143821	1	409105	5	NULL	NULL	0	NULL	change 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The change in AT1-R mRNA level was less rapid than that in response to activation of phosphoinositidase C by Ang II or adenylyl cyclase by forskolin or by dibutyryl-cAMP .
	manualset3
143822	2	409105	5	NULL	NULL	0	NULL	AT1-R mRNA level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The change in AT1-R mRNA level was less rapid than that in response to activation of phosphoinositidase C by Ang II or adenylyl cyclase by forskolin or by dibutyryl-cAMP .
	manualset3
143823	3	409105	5	NULL	NULL	0	NULL	response 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The change in AT1-R mRNA level was less rapid than that in response to activation of phosphoinositidase C by Ang II or adenylyl cyclase by forskolin or by dibutyryl-cAMP .
	manualset3
143824	4	409105	5	NULL	NULL	NULL	NULL	activation 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The change in AT1-R mRNA level was less rapid than that in response to activation of phosphoinositidase C by Ang II or adenylyl cyclase by forskolin or by dibutyryl-cAMP .
	manualset3
143825	5	409105	5	NULL	NULL	0	NULL	phosphoinositidase C	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The change in AT1-R mRNA level was less rapid than that in response to activation of phosphoinositidase C by Ang II or adenylyl cyclase by forskolin or by dibutyryl-cAMP .
	manualset3
143826	6	409105	5	NULL	NULL	0	NULL	Ang II 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The change in AT1-R mRNA level was less rapid than that in response to activation of phosphoinositidase C by Ang II or adenylyl cyclase by forskolin or by dibutyryl-cAMP .
	manualset3
143827	7	409105	5	NULL	NULL	0	NULL	adenylyl cyclase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The change in AT1-R mRNA level was less rapid than that in response to activation of phosphoinositidase C by Ang II or adenylyl cyclase by forskolin or by dibutyryl-cAMP .
	manualset3
143828	8	409105	5	NULL	NULL	0	NULL	forskolin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The change in AT1-R mRNA level was less rapid than that in response to activation of phosphoinositidase C by Ang II or adenylyl cyclase by forskolin or by dibutyryl-cAMP .
	manualset3
143829	9	409105	5	NULL	NULL	0	NULL	dibutyryl-cAMP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The change in AT1-R mRNA level was less rapid than that in response to activation of phosphoinositidase C by Ang II or adenylyl cyclase by forskolin or by dibutyryl-cAMP .
	manualset3
143830	1	409106	5	NULL	NULL	0	NULL	change 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The change in pattern of serum cholesterol was parallel to the change in serum AFP .
	manualset3
143831	2	409106	5	NULL	NULL	0	NULL	pattern 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The change in pattern of serum cholesterol was parallel to the change in serum AFP .
	manualset3
143832	3	409106	5	NULL	NULL	0	NULL	serum cholesterol 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The change in pattern of serum cholesterol was parallel to the change in serum AFP .
	manualset3
143833	4	409106	5	NULL	NULL	0	NULL	change 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The change in pattern of serum cholesterol was parallel to the change in serum AFP .
	manualset3
143834	5	409106	5	NULL	NULL	0	NULL	serum AFP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The change in pattern of serum cholesterol was parallel to the change in serum AFP .
	manualset3
143835	1	409107	5	NULL	NULL	0	NULL	change 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The change of this single residue from lysine to glutamine resulted in a prolonged half life of CYS3 and impaired responsiveness of CYS3 degradation to sulfur level changes .
	manualset3
143836	2	409107	5	NULL	NULL	0	NULL	single residue	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The change of this single residue from lysine to glutamine resulted in a prolonged half life of CYS3 and impaired responsiveness of CYS3 degradation to sulfur level changes .
	manualset3
143837	3	409107	5	NULL	NULL	0	NULL	lysine 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The change of this single residue from lysine to glutamine resulted in a prolonged half life of CYS3 and impaired responsiveness of CYS3 degradation to sulfur level changes .
	manualset3
143838	4	409107	5	NULL	NULL	0	NULL	glutamine 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The change of this single residue from lysine to glutamine resulted in a prolonged half life of CYS3 and impaired responsiveness of CYS3 degradation to sulfur level changes .
	manualset3
143839	5	409107	5	NULL	NULL	0	NULL	half life 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The change of this single residue from lysine to glutamine resulted in a prolonged half life of CYS3 and impaired responsiveness of CYS3 degradation to sulfur level changes .
	manualset3
143840	6	409107	5	NULL	NULL	0	NULL	CYS3 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The change of this single residue from lysine to glutamine resulted in a prolonged half life of CYS3 and impaired responsiveness of CYS3 degradation to sulfur level changes .
	manualset3
143841	7	409107	5	NULL	NULL	0	NULL	impaired responsiveness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The change of this single residue from lysine to glutamine resulted in a prolonged half life of CYS3 and impaired responsiveness of CYS3 degradation to sulfur level changes .
	manualset3
143842	8	409107	5	NULL	NULL	0	NULL	CYS3 degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The change of this single residue from lysine to glutamine resulted in a prolonged half life of CYS3 and impaired responsiveness of CYS3 degradation to sulfur level changes .
	manualset3
143843	9	409107	5	NULL	NULL	0	NULL	sulfur level changes 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The change of this single residue from lysine to glutamine resulted in a prolonged half life of CYS3 and impaired responsiveness of CYS3 degradation to sulfur level changes .
	manualset3
143844	1	409108	5	NULL	NULL	0	NULL	changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The changes in casein micelle size were poorly correlated with the level of whey protein denaturation .
	manualset3
143845	2	409108	5	NULL	NULL	0	NULL	casein micelle size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The changes in casein micelle size were poorly correlated with the level of whey protein denaturation .
	manualset3
143846	3	409108	5	NULL	NULL	0	NULL	level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The changes in casein micelle size were poorly correlated with the level of whey protein denaturation .
	manualset3
143847	4	409108	5	NULL	NULL	0	NULL	whey protein denaturation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The changes in casein micelle size were poorly correlated with the level of whey protein denaturation .
	manualset3
143848	1	409109	5	NULL	NULL	0	NULL	set 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A set of 18 Alu markers and three short tandem repeats ( STRs ) closely linked to the CD4 , F13B and DM Alu have been analyzed in seven samples from Majorca , Corsica , Sardinia and Sicily to explore some of these issues .
	manualset3
143849	2	409109	5	NULL	NULL	0	NULL	18 Alu markers	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A set of 18 Alu markers and three short tandem repeats ( STRs ) closely linked to the CD4 , F13B and DM Alu have been analyzed in seven samples from Majorca , Corsica , Sardinia and Sicily to explore some of these issues .
	manualset3
143850	3	409109	5	NULL	NULL	0	NULL	three 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A set of 18 Alu markers and three short tandem repeats ( STRs ) closely linked to the CD4 , F13B and DM Alu have been analyzed in seven samples from Majorca , Corsica , Sardinia and Sicily to explore some of these issues .
	manualset3
143851	4	409109	5	NULL	NULL	0	NULL	short tandem repeats ( STRs ) 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A set of 18 Alu markers and three short tandem repeats ( STRs ) closely linked to the CD4 , F13B and DM Alu have been analyzed in seven samples from Majorca , Corsica , Sardinia and Sicily to explore some of these issues .
	manualset3
143852	5	409109	5	NULL	NULL	0	NULL	CD4 Alu	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A set of 18 Alu markers and three short tandem repeats ( STRs ) closely linked to the CD4 , F13B and DM Alu have been analyzed in seven samples from Majorca , Corsica , Sardinia and Sicily to explore some of these issues .
	manualset3
143853	6	409109	5	NULL	NULL	0	NULL	F13B Alu	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A set of 18 Alu markers and three short tandem repeats ( STRs ) closely linked to the CD4 , F13B and DM Alu have been analyzed in seven samples from Majorca , Corsica , Sardinia and Sicily to explore some of these issues .
	manualset3
143854	7	409109	5	NULL	NULL	0	NULL	DM Alu	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A set of 18 Alu markers and three short tandem repeats ( STRs ) closely linked to the CD4 , F13B and DM Alu have been analyzed in seven samples from Majorca , Corsica , Sardinia and Sicily to explore some of these issues .
	manualset3
143855	8	409109	5	NULL	NULL	0	NULL	seven samples	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A set of 18 Alu markers and three short tandem repeats ( STRs ) closely linked to the CD4 , F13B and DM Alu have been analyzed in seven samples from Majorca , Corsica , Sardinia and Sicily to explore some of these issues .
	manualset3
143856	9	409109	5	NULL	NULL	0	NULL	Majorca 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A set of 18 Alu markers and three short tandem repeats ( STRs ) closely linked to the CD4 , F13B and DM Alu have been analyzed in seven samples from Majorca , Corsica , Sardinia and Sicily to explore some of these issues .
	manualset3
143857	10	409109	5	NULL	NULL	0	NULL	Corsica 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A set of 18 Alu markers and three short tandem repeats ( STRs ) closely linked to the CD4 , F13B and DM Alu have been analyzed in seven samples from Majorca , Corsica , Sardinia and Sicily to explore some of these issues .
	manualset3
143858	11	409109	5	NULL	NULL	0	NULL	Sardinia 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A set of 18 Alu markers and three short tandem repeats ( STRs ) closely linked to the CD4 , F13B and DM Alu have been analyzed in seven samples from Majorca , Corsica , Sardinia and Sicily to explore some of these issues .
	manualset3
143859	12	409109	5	NULL	NULL	0	NULL	Sicily 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A set of 18 Alu markers and three short tandem repeats ( STRs ) closely linked to the CD4 , F13B and DM Alu have been analyzed in seven samples from Majorca , Corsica , Sardinia and Sicily to explore some of these issues .
	manualset3
143860	13	409109	5	NULL	NULL	0	NULL	issues 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A set of 18 Alu markers and three short tandem repeats ( STRs ) closely linked to the CD4 , F13B and DM Alu have been analyzed in seven samples from Majorca , Corsica , Sardinia and Sicily to explore some of these issues .
	manualset3
143861	1	409110	5	NULL	NULL	0	NULL	chaperonin GroEL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The chaperonin GroEL and its cofactor GroES facilitate protein folding in an ATP-regulated manner .
	manualset3
143862	2	409110	5	NULL	NULL	0	NULL	cofactor GroES 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The chaperonin GroEL and its cofactor GroES facilitate protein folding in an ATP-regulated manner .
	manualset3
143863	3	409110	5	NULL	NULL	0	NULL	protein folding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The chaperonin GroEL and its cofactor GroES facilitate protein folding in an ATP-regulated manner .
	manualset3
143864	4	409110	5	NULL	NULL	0	NULL	ATP-regulated manner	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The chaperonin GroEL and its cofactor GroES facilitate protein folding in an ATP-regulated manner .
	manualset3
143865	1	409111	5	NULL	NULL	0	NULL	characteristics 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The characteristics of excitement is cybotaxis discharge .
	manualset3
143866	2	409111	5	NULL	NULL	0	NULL	excitement 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The characteristics of excitement is cybotaxis discharge .
	manualset3
143867	3	409111	5	NULL	NULL	0	NULL	cybotaxis discharge 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The characteristics of excitement is cybotaxis discharge .
	manualset3
143868	1	409112	5	NULL	NULL	0	NULL	charged current 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The charged current on the gas sensor was enhanced when the ZnO single-crystal wire was exposed to a H2S stream .
	manualset3
143869	2	409112	5	NULL	NULL	0	NULL	gas sensor	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The charged current on the gas sensor was enhanced when the ZnO single-crystal wire was exposed to a H2S stream .
	manualset3
143870	3	409112	5	NULL	NULL	0	NULL	ZnO single-crystal wire 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The charged current on the gas sensor was enhanced when the ZnO single-crystal wire was exposed to a H2S stream .
	manualset3
143871	4	409112	5	NULL	NULL	0	NULL	H2S stream	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The charged current on the gas sensor was enhanced when the ZnO single-crystal wire was exposed to a H2S stream .
	manualset3
143872	1	409113	5	NULL	NULL	0	NULL	charged groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The charged groups at the interface of some blood cells .
	manualset3
143873	2	409113	5	NULL	NULL	0	NULL	interface 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The charged groups at the interface of some blood cells .
	manualset3
143874	3	409113	5	NULL	NULL	0	NULL	blood cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The charged groups at the interface of some blood cells .
	manualset3
143875	1	409114	5	NULL	NULL	0	NULL	charged hydrogels	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The charged hydrogels display strong electrostatic interactions with the appropriate cationic or anionic porphyrins to give materials which are intended to be used to generate cytotoxic singlet oxygen ( 1O2 ) on photoexcitation and can therefore be used to reduce postoperative infection of the intraocular hydrogel-based replacement lenses that are used in cataract surgery .
	manualset3
143876	2	409114	5	NULL	NULL	0	NULL	strong electrostatic interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The charged hydrogels display strong electrostatic interactions with the appropriate cationic or anionic porphyrins to give materials which are intended to be used to generate cytotoxic singlet oxygen ( 1O2 ) on photoexcitation and can therefore be used to reduce postoperative infection of the intraocular hydrogel-based replacement lenses that are used in cataract surgery .
	manualset3
143877	3	409114	5	NULL	NULL	0	NULL	cationic or anionic porphyrins	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The charged hydrogels display strong electrostatic interactions with the appropriate cationic or anionic porphyrins to give materials which are intended to be used to generate cytotoxic singlet oxygen ( 1O2 ) on photoexcitation and can therefore be used to reduce postoperative infection of the intraocular hydrogel-based replacement lenses that are used in cataract surgery .
	manualset3
143878	4	409114	5	NULL	NULL	0	NULL	materials 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The charged hydrogels display strong electrostatic interactions with the appropriate cationic or anionic porphyrins to give materials which are intended to be used to generate cytotoxic singlet oxygen ( 1O2 ) on photoexcitation and can therefore be used to reduce postoperative infection of the intraocular hydrogel-based replacement lenses that are used in cataract surgery .
	manualset3
143879	5	409114	5	NULL	NULL	0	NULL	cytotoxic singlet oxygen ( 1O2 )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The charged hydrogels display strong electrostatic interactions with the appropriate cationic or anionic porphyrins to give materials which are intended to be used to generate cytotoxic singlet oxygen ( 1O2 ) on photoexcitation and can therefore be used to reduce postoperative infection of the intraocular hydrogel-based replacement lenses that are used in cataract surgery .
	manualset3
143880	6	409114	5	NULL	NULL	0	NULL	photoexcitation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The charged hydrogels display strong electrostatic interactions with the appropriate cationic or anionic porphyrins to give materials which are intended to be used to generate cytotoxic singlet oxygen ( 1O2 ) on photoexcitation and can therefore be used to reduce postoperative infection of the intraocular hydrogel-based replacement lenses that are used in cataract surgery .
	manualset3
143881	7	409114	5	NULL	NULL	0	NULL	postoperative infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The charged hydrogels display strong electrostatic interactions with the appropriate cationic or anionic porphyrins to give materials which are intended to be used to generate cytotoxic singlet oxygen ( 1O2 ) on photoexcitation and can therefore be used to reduce postoperative infection of the intraocular hydrogel-based replacement lenses that are used in cataract surgery .
	manualset3
143882	8	409114	5	NULL	NULL	0	NULL	intraocular hydrogel-based replacement lenses	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The charged hydrogels display strong electrostatic interactions with the appropriate cationic or anionic porphyrins to give materials which are intended to be used to generate cytotoxic singlet oxygen ( 1O2 ) on photoexcitation and can therefore be used to reduce postoperative infection of the intraocular hydrogel-based replacement lenses that are used in cataract surgery .
	manualset3
143883	9	409114	5	NULL	NULL	0	NULL	cataract surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The charged hydrogels display strong electrostatic interactions with the appropriate cationic or anionic porphyrins to give materials which are intended to be used to generate cytotoxic singlet oxygen ( 1O2 ) on photoexcitation and can therefore be used to reduce postoperative infection of the intraocular hydrogel-based replacement lenses that are used in cataract surgery .
	manualset3
143884	1	409115	5	NULL	NULL	0	NULL	chemical complexity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemical and anatomical complexity of this region suggests that other neurotransmitter systems and neuronal circuits within and extending from the basal ganglia may be disturbed in the pathogenesis of TD .
	manualset3
143885	2	409115	5	NULL	NULL	0	NULL	anatomical complexity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemical and anatomical complexity of this region suggests that other neurotransmitter systems and neuronal circuits within and extending from the basal ganglia may be disturbed in the pathogenesis of TD .
	manualset3
143886	3	409115	5	NULL	NULL	0	NULL	region 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemical and anatomical complexity of this region suggests that other neurotransmitter systems and neuronal circuits within and extending from the basal ganglia may be disturbed in the pathogenesis of TD .
	manualset3
143887	4	409115	5	NULL	NULL	0	NULL	neurotransmitter systems	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemical and anatomical complexity of this region suggests that other neurotransmitter systems and neuronal circuits within and extending from the basal ganglia may be disturbed in the pathogenesis of TD .
	manualset3
143888	5	409115	5	NULL	NULL	0	NULL	neuronal circuits	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemical and anatomical complexity of this region suggests that other neurotransmitter systems and neuronal circuits within and extending from the basal ganglia may be disturbed in the pathogenesis of TD .
	manualset3
143889	6	409115	5	NULL	NULL	0	NULL	basal ganglia	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemical and anatomical complexity of this region suggests that other neurotransmitter systems and neuronal circuits within and extending from the basal ganglia may be disturbed in the pathogenesis of TD .
	manualset3
143890	7	409115	5	NULL	NULL	0	NULL	pathogenesis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemical and anatomical complexity of this region suggests that other neurotransmitter systems and neuronal circuits within and extending from the basal ganglia may be disturbed in the pathogenesis of TD .
	manualset3
143891	8	409115	5	NULL	NULL	0	NULL	TD 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemical and anatomical complexity of this region suggests that other neurotransmitter systems and neuronal circuits within and extending from the basal ganglia may be disturbed in the pathogenesis of TD .
	manualset3
143892	1	409116	5	NULL	NULL	0	NULL	chemical composition	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemical composition of the membranes of protoplasts and L-forms of Staphylococcus aureus .
	manualset3
143893	2	409116	5	NULL	NULL	0	NULL	membranes 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemical composition of the membranes of protoplasts and L-forms of Staphylococcus aureus .
	manualset3
143894	3	409116	5	NULL	NULL	0	NULL	protoplasts 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemical composition of the membranes of protoplasts and L-forms of Staphylococcus aureus .
	manualset3
143895	4	409116	5	NULL	NULL	0	NULL	L-forms of Staphylococcus aureus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemical composition of the membranes of protoplasts and L-forms of Staphylococcus aureus .
	manualset3
143896	1	409117	5	NULL	NULL	0	NULL	chemotherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemotherapy consisted of mAMSA ( 100 mg/m2 per day i.v. , days 1-3 ) , ARA-C ( 100 mg/m2 , twice daily , days 1-6 ) , and VP 16 ( 150 mg/m2 per day , days 4-6 ) .
	manualset3
143897	2	409117	5	NULL	NULL	0	NULL	mAMSA 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemotherapy consisted of mAMSA ( 100 mg/m2 per day i.v. , days 1-3 ) , ARA-C ( 100 mg/m2 , twice daily , days 1-6 ) , and VP 16 ( 150 mg/m2 per day , days 4-6 ) .
	manualset3
143898	3	409117	5	NULL	NULL	0	NULL	100 mg/m2 per day i.v. 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemotherapy consisted of mAMSA ( 100 mg/m2 per day i.v. , days 1-3 ) , ARA-C ( 100 mg/m2 , twice daily , days 1-6 ) , and VP 16 ( 150 mg/m2 per day , days 4-6 ) .
	manualset3
143899	4	409117	5	NULL	NULL	0	NULL	days 1-3	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemotherapy consisted of mAMSA ( 100 mg/m2 per day i.v. , days 1-3 ) , ARA-C ( 100 mg/m2 , twice daily , days 1-6 ) , and VP 16 ( 150 mg/m2 per day , days 4-6 ) .
	manualset3
143900	5	409117	5	NULL	NULL	0	NULL	ARA-C	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemotherapy consisted of mAMSA ( 100 mg/m2 per day i.v. , days 1-3 ) , ARA-C ( 100 mg/m2 , twice daily , days 1-6 ) , and VP 16 ( 150 mg/m2 per day , days 4-6 ) .
	manualset3
143901	6	409117	5	NULL	NULL	0	NULL	100 mg/m2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemotherapy consisted of mAMSA ( 100 mg/m2 per day i.v. , days 1-3 ) , ARA-C ( 100 mg/m2 , twice daily , days 1-6 ) , and VP 16 ( 150 mg/m2 per day , days 4-6 ) .
	manualset3
143902	7	409117	5	NULL	NULL	0	NULL	days 1-6 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemotherapy consisted of mAMSA ( 100 mg/m2 per day i.v. , days 1-3 ) , ARA-C ( 100 mg/m2 , twice daily , days 1-6 ) , and VP 16 ( 150 mg/m2 per day , days 4-6 ) .
	manualset3
143903	8	409117	5	NULL	NULL	0	NULL	VP 16	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemotherapy consisted of mAMSA ( 100 mg/m2 per day i.v. , days 1-3 ) , ARA-C ( 100 mg/m2 , twice daily , days 1-6 ) , and VP 16 ( 150 mg/m2 per day , days 4-6 ) .
	manualset3
143904	9	409117	5	NULL	NULL	0	NULL	150 mg/m2 per day	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemotherapy consisted of mAMSA ( 100 mg/m2 per day i.v. , days 1-3 ) , ARA-C ( 100 mg/m2 , twice daily , days 1-6 ) , and VP 16 ( 150 mg/m2 per day , days 4-6 ) .
	manualset3
143905	10	409117	5	NULL	NULL	0	NULL	days 4-6	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemotherapy consisted of mAMSA ( 100 mg/m2 per day i.v. , days 1-3 ) , ARA-C ( 100 mg/m2 , twice daily , days 1-6 ) , and VP 16 ( 150 mg/m2 per day , days 4-6 ) .
	manualset3
143906	1	409118	5	NULL	NULL	0	NULL	childhood obesity epidemic	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The childhood obesity epidemic is expected to increase cardiovascular disease risk , but the impact of obesity on vascular function in children is not fully understood .
	manualset3
143907	2	409118	5	NULL	NULL	0	NULL	cardiovascular disease risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The childhood obesity epidemic is expected to increase cardiovascular disease risk , but the impact of obesity on vascular function in children is not fully understood .
	manualset3
143908	3	409118	5	NULL	NULL	0	NULL	impact 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The childhood obesity epidemic is expected to increase cardiovascular disease risk , but the impact of obesity on vascular function in children is not fully understood .
	manualset3
143909	4	409118	5	NULL	NULL	0	NULL	obesity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The childhood obesity epidemic is expected to increase cardiovascular disease risk , but the impact of obesity on vascular function in children is not fully understood .
	manualset3
143910	5	409118	5	NULL	NULL	0	NULL	vascular function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The childhood obesity epidemic is expected to increase cardiovascular disease risk , but the impact of obesity on vascular function in children is not fully understood .
	manualset3
143911	6	409118	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The childhood obesity epidemic is expected to increase cardiovascular disease risk , but the impact of obesity on vascular function in children is not fully understood .
	manualset3
143912	1	409119	5	NULL	NULL	0	NULL	chimeric genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The chimeric genes contained a 5 ' splicing site ( SS ) from SV40 and a 3 ' SS from the inserted gene .
	manualset3
143913	2	409119	5	NULL	NULL	0	NULL	5 ' splicing site ( SS ) 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The chimeric genes contained a 5 ' splicing site ( SS ) from SV40 and a 3 ' SS from the inserted gene .
	manualset3
143914	3	409119	5	NULL	NULL	0	NULL	SV40	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The chimeric genes contained a 5 ' splicing site ( SS ) from SV40 and a 3 ' SS from the inserted gene .
	manualset3
143915	4	409119	5	NULL	NULL	0	NULL	3 ' SS 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The chimeric genes contained a 5 ' splicing site ( SS ) from SV40 and a 3 ' SS from the inserted gene .
	manualset3
143916	5	409119	5	NULL	NULL	0	NULL	inserted gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The chimeric genes contained a 5 ' splicing site ( SS ) from SV40 and a 3 ' SS from the inserted gene .
	manualset3
143917	1	409120	5	NULL	NULL	0	NULL	chiral recognition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The chiral recognition of the selected aromatic chiral compounds by native beta-cyclodextrin ( beta-CD ) based on bimodal complexation was studied using a flexible docking algorithm FDOCK .
	manualset3
143918	2	409120	5	NULL	NULL	0	NULL	selected aromatic chiral compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The chiral recognition of the selected aromatic chiral compounds by native beta-cyclodextrin ( beta-CD ) based on bimodal complexation was studied using a flexible docking algorithm FDOCK .
	manualset3
143919	3	409120	5	NULL	NULL	0	NULL	native beta-cyclodextrin ( beta-CD ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The chiral recognition of the selected aromatic chiral compounds by native beta-cyclodextrin ( beta-CD ) based on bimodal complexation was studied using a flexible docking algorithm FDOCK .
	manualset3
143920	4	409120	5	NULL	NULL	0	NULL	bimodal complexation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The chiral recognition of the selected aromatic chiral compounds by native beta-cyclodextrin ( beta-CD ) based on bimodal complexation was studied using a flexible docking algorithm FDOCK .
	manualset3
143921	5	409120	5	NULL	NULL	0	NULL	flexible docking algorithm FDOCK	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The chiral recognition of the selected aromatic chiral compounds by native beta-cyclodextrin ( beta-CD ) based on bimodal complexation was studied using a flexible docking algorithm FDOCK .
	manualset3
143922	1	409121	5	NULL	NULL	0	NULL	cholesterol-lowering effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cholesterol-lowering effect of coconut flakes in humans with moderately raised serum cholesterol .
	manualset3
143923	2	409121	5	NULL	NULL	0	NULL	coconut flakes	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The cholesterol-lowering effect of coconut flakes in humans with moderately raised serum cholesterol .
	manualset3
143924	3	409121	5	NULL	NULL	0	NULL	humans 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The cholesterol-lowering effect of coconut flakes in humans with moderately raised serum cholesterol .
	manualset3
143925	4	409121	5	NULL	NULL	0	NULL	serum cholesterol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The cholesterol-lowering effect of coconut flakes in humans with moderately raised serum cholesterol .
	manualset3
143926	1	409122	5	NULL	NULL	0	NULL	seven-base-pair deletion	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A seven-base-pair deletion in an intron of the albumin gene of analbuminemic rats .
	manualset3
143927	2	409122	5	NULL	NULL	0	NULL	intron 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A seven-base-pair deletion in an intron of the albumin gene of analbuminemic rats .
	manualset3
143928	3	409122	5	NULL	NULL	0	NULL	albumin gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A seven-base-pair deletion in an intron of the albumin gene of analbuminemic rats .
	manualset3
143929	4	409122	5	NULL	NULL	0	NULL	analbuminemic rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A seven-base-pair deletion in an intron of the albumin gene of analbuminemic rats .
	manualset3
143930	1	409123	5	NULL	NULL	0	NULL	chondrocyte K + channel	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The chondrocyte K + channel may contribute to the unusually high ( K + ) found in the extracellular fluid of growth plate cartilage .
	manualset3
143931	2	409123	5	NULL	NULL	0	NULL	( K + )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The chondrocyte K + channel may contribute to the unusually high ( K + ) found in the extracellular fluid of growth plate cartilage .
	manualset3
143932	3	409123	5	NULL	NULL	0	NULL	extracellular fluid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The chondrocyte K + channel may contribute to the unusually high ( K + ) found in the extracellular fluid of growth plate cartilage .
	manualset3
143933	4	409123	5	NULL	NULL	0	NULL	growth plate cartilage	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The chondrocyte K + channel may contribute to the unusually high ( K + ) found in the extracellular fluid of growth plate cartilage .
	manualset3
143934	1	409124	5	NULL	NULL	0	NULL	chromatographic separation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The chromatographic separation was performed on a Nucleosil C18 , 5 microm ( 150x1 mm I.D. ) column , using a gradient of acetonitrile in 5 mM ammonium formate , pH 3.0 as the mobile phase , delivered at a flow-rate of 50 microl/min .
	manualset3
143935	2	409124	5	NULL	NULL	0	NULL	Nucleosil C18 , 5 microm ( 150x1 mm I.D. ) column	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The chromatographic separation was performed on a Nucleosil C18 , 5 microm ( 150x1 mm I.D. ) column , using a gradient of acetonitrile in 5 mM ammonium formate , pH 3.0 as the mobile phase , delivered at a flow-rate of 50 microl/min .
	manualset3
143936	3	409124	5	NULL	NULL	0	NULL	gradient 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The chromatographic separation was performed on a Nucleosil C18 , 5 microm ( 150x1 mm I.D. ) column , using a gradient of acetonitrile in 5 mM ammonium formate , pH 3.0 as the mobile phase , delivered at a flow-rate of 50 microl/min .
	manualset3
143937	4	409124	5	NULL	NULL	0	NULL	acetonitrile 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The chromatographic separation was performed on a Nucleosil C18 , 5 microm ( 150x1 mm I.D. ) column , using a gradient of acetonitrile in 5 mM ammonium formate , pH 3.0 as the mobile phase , delivered at a flow-rate of 50 microl/min .
	manualset3
143938	5	409124	5	NULL	NULL	0	NULL	5 mM ammonium formate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The chromatographic separation was performed on a Nucleosil C18 , 5 microm ( 150x1 mm I.D. ) column , using a gradient of acetonitrile in 5 mM ammonium formate , pH 3.0 as the mobile phase , delivered at a flow-rate of 50 microl/min .
	manualset3
143939	6	409124	5	NULL	NULL	0	NULL	pH 3.0 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The chromatographic separation was performed on a Nucleosil C18 , 5 microm ( 150x1 mm I.D. ) column , using a gradient of acetonitrile in 5 mM ammonium formate , pH 3.0 as the mobile phase , delivered at a flow-rate of 50 microl/min .
	manualset3
143940	7	409124	5	NULL	NULL	0	NULL	mobile phase	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The chromatographic separation was performed on a Nucleosil C18 , 5 microm ( 150x1 mm I.D. ) column , using a gradient of acetonitrile in 5 mM ammonium formate , pH 3.0 as the mobile phase , delivered at a flow-rate of 50 microl/min .
	manualset3
143941	8	409124	5	NULL	NULL	0	NULL	flow-rate 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The chromatographic separation was performed on a Nucleosil C18 , 5 microm ( 150x1 mm I.D. ) column , using a gradient of acetonitrile in 5 mM ammonium formate , pH 3.0 as the mobile phase , delivered at a flow-rate of 50 microl/min .
	manualset3
143942	9	409124	5	NULL	NULL	0	NULL	50 microl/min	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The chromatographic separation was performed on a Nucleosil C18 , 5 microm ( 150x1 mm I.D. ) column , using a gradient of acetonitrile in 5 mM ammonium formate , pH 3.0 as the mobile phase , delivered at a flow-rate of 50 microl/min .
	manualset3
143943	1	409125	5	NULL	NULL	0	NULL	chromosomal location	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The chromosomal location of each aspartyl proteinase has been determined by a variety of gene mapping methods employing recombinant DNA probes including ; analysis of somatic cell hybrid mapping panels , in situ hybridization to metaphase chromosome preparations and family linkage analysis with polymorphic markers .
	manualset3
143944	2	409125	5	NULL	NULL	0	NULL	aspartyl proteinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The chromosomal location of each aspartyl proteinase has been determined by a variety of gene mapping methods employing recombinant DNA probes including ; analysis of somatic cell hybrid mapping panels , in situ hybridization to metaphase chromosome preparations and family linkage analysis with polymorphic markers .
	manualset3
143945	3	409125	5	NULL	NULL	0	NULL	gene mapping methods 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The chromosomal location of each aspartyl proteinase has been determined by a variety of gene mapping methods employing recombinant DNA probes including ; analysis of somatic cell hybrid mapping panels , in situ hybridization to metaphase chromosome preparations and family linkage analysis with polymorphic markers .
	manualset3
143946	4	409125	5	NULL	NULL	0	NULL	recombinant DNA probes 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The chromosomal location of each aspartyl proteinase has been determined by a variety of gene mapping methods employing recombinant DNA probes including ; analysis of somatic cell hybrid mapping panels , in situ hybridization to metaphase chromosome preparations and family linkage analysis with polymorphic markers .
	manualset3
143947	5	409125	5	NULL	NULL	0	NULL	analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The chromosomal location of each aspartyl proteinase has been determined by a variety of gene mapping methods employing recombinant DNA probes including ; analysis of somatic cell hybrid mapping panels , in situ hybridization to metaphase chromosome preparations and family linkage analysis with polymorphic markers .
	manualset3
143948	6	409125	5	NULL	NULL	0	NULL	somatic cell hybrid mapping panels	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The chromosomal location of each aspartyl proteinase has been determined by a variety of gene mapping methods employing recombinant DNA probes including ; analysis of somatic cell hybrid mapping panels , in situ hybridization to metaphase chromosome preparations and family linkage analysis with polymorphic markers .
	manualset3
143949	7	409125	5	NULL	NULL	0	NULL	in situ hybridization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The chromosomal location of each aspartyl proteinase has been determined by a variety of gene mapping methods employing recombinant DNA probes including ; analysis of somatic cell hybrid mapping panels , in situ hybridization to metaphase chromosome preparations and family linkage analysis with polymorphic markers .
	manualset3
143950	8	409125	5	NULL	NULL	0	NULL	metaphase chromosome preparations	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The chromosomal location of each aspartyl proteinase has been determined by a variety of gene mapping methods employing recombinant DNA probes including ; analysis of somatic cell hybrid mapping panels , in situ hybridization to metaphase chromosome preparations and family linkage analysis with polymorphic markers .
	manualset3
143951	9	409125	5	NULL	NULL	0	NULL	family linkage analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The chromosomal location of each aspartyl proteinase has been determined by a variety of gene mapping methods employing recombinant DNA probes including ; analysis of somatic cell hybrid mapping panels , in situ hybridization to metaphase chromosome preparations and family linkage analysis with polymorphic markers .
	manualset3
143952	10	409125	5	NULL	NULL	0	NULL	polymorphic markers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The chromosomal location of each aspartyl proteinase has been determined by a variety of gene mapping methods employing recombinant DNA probes including ; analysis of somatic cell hybrid mapping panels , in situ hybridization to metaphase chromosome preparations and family linkage analysis with polymorphic markers .
	manualset3
143953	1	409126	5	NULL	NULL	0	NULL	chronic toxicity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The chronic toxicity of chloroquine ( SN 7618 ) .
	manualset3
143954	2	409126	5	NULL	NULL	0	NULL	chloroquine ( SN 7618 )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The chronic toxicity of chloroquine ( SN 7618 ) .
	manualset3
143955	1	409127	5	NULL	NULL	0	NULL	chronic use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The chronic use of phenothiazine is known to result in ventricular arrhythmias in certain patients .
	manualset3
143956	2	409127	5	NULL	NULL	0	NULL	phenothiazine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The chronic use of phenothiazine is known to result in ventricular arrhythmias in certain patients .
	manualset3
143957	3	409127	5	NULL	NULL	0	NULL	result 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The chronic use of phenothiazine is known to result in ventricular arrhythmias in certain patients .
	manualset3
143958	4	409127	5	NULL	NULL	0	NULL	ventricular arrhythmias	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The chronic use of phenothiazine is known to result in ventricular arrhythmias in certain patients .
	manualset3
143959	5	409127	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The chronic use of phenothiazine is known to result in ventricular arrhythmias in certain patients .
	manualset3
143960	1	409128	5	NULL	NULL	0	NULL	ciliated protozoan Cryptocaryon irritans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The ciliated protozoan Cryptocaryon irritans , a parasite of seawater fishes , was found to express an antigen that elicits antibodies in rabbits and tiger puffer ( Takifugu ruburipes ) .
	manualset3
143961	2	409128	5	NULL	NULL	0	NULL	parasite 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The ciliated protozoan Cryptocaryon irritans , a parasite of seawater fishes , was found to express an antigen that elicits antibodies in rabbits and tiger puffer ( Takifugu ruburipes ) .
	manualset3
143962	3	409128	5	NULL	NULL	0	NULL	seawater fishes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The ciliated protozoan Cryptocaryon irritans , a parasite of seawater fishes , was found to express an antigen that elicits antibodies in rabbits and tiger puffer ( Takifugu ruburipes ) .
	manualset3
143963	4	409128	5	NULL	NULL	0	NULL	antigen 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The ciliated protozoan Cryptocaryon irritans , a parasite of seawater fishes , was found to express an antigen that elicits antibodies in rabbits and tiger puffer ( Takifugu ruburipes ) .
	manualset3
143964	5	409128	5	NULL	NULL	0	NULL	antibodies 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The ciliated protozoan Cryptocaryon irritans , a parasite of seawater fishes , was found to express an antigen that elicits antibodies in rabbits and tiger puffer ( Takifugu ruburipes ) .
	manualset3
143965	6	409128	5	NULL	NULL	0	NULL	rabbits 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The ciliated protozoan Cryptocaryon irritans , a parasite of seawater fishes , was found to express an antigen that elicits antibodies in rabbits and tiger puffer ( Takifugu ruburipes ) .
	manualset3
143966	7	409128	5	NULL	NULL	0	NULL	tiger puffer ( Takifugu ruburipes )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The ciliated protozoan Cryptocaryon irritans , a parasite of seawater fishes , was found to express an antigen that elicits antibodies in rabbits and tiger puffer ( Takifugu ruburipes ) .
	manualset3
143967	1	409129	5	NULL	NULL	0	NULL	circadian clock	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The circadian clock is an endogenous oscillator with a period of approximately 24 h that allows organisms to anticipate , and respond to , changes in the environment .
	manualset3
143968	2	409129	5	NULL	NULL	0	NULL	endogenous oscillator	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The circadian clock is an endogenous oscillator with a period of approximately 24 h that allows organisms to anticipate , and respond to , changes in the environment .
	manualset3
143969	3	409129	5	NULL	NULL	0	NULL	period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The circadian clock is an endogenous oscillator with a period of approximately 24 h that allows organisms to anticipate , and respond to , changes in the environment .
	manualset3
143970	4	409129	5	NULL	NULL	0	NULL	24 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The circadian clock is an endogenous oscillator with a period of approximately 24 h that allows organisms to anticipate , and respond to , changes in the environment .
	manualset3
143971	5	409129	5	NULL	NULL	0	NULL	organisms 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The circadian clock is an endogenous oscillator with a period of approximately 24 h that allows organisms to anticipate , and respond to , changes in the environment .
	manualset3
143972	6	409129	5	NULL	NULL	0	NULL	changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The circadian clock is an endogenous oscillator with a period of approximately 24 h that allows organisms to anticipate , and respond to , changes in the environment .
	manualset3
143973	7	409129	5	NULL	NULL	0	NULL	environment 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The circadian clock is an endogenous oscillator with a period of approximately 24 h that allows organisms to anticipate , and respond to , changes in the environment .
	manualset3
143974	1	409130	5	NULL	NULL	0	NULL	environment 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The circadian clock located in the suprachiasmatic nuclei ( SCN ) of the hypothalamus regulates daily temporal organization in behavior and neuroendocrine function .
	manualset3
143975	2	409130	5	NULL	NULL	0	NULL	suprachiasmatic nuclei ( SCN ) 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The circadian clock located in the suprachiasmatic nuclei ( SCN ) of the hypothalamus regulates daily temporal organization in behavior and neuroendocrine function .
	manualset3
143976	3	409130	5	NULL	NULL	0	NULL	hypothalamus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The circadian clock located in the suprachiasmatic nuclei ( SCN ) of the hypothalamus regulates daily temporal organization in behavior and neuroendocrine function .
	manualset3
143977	4	409130	5	NULL	NULL	0	NULL	temporal organization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The circadian clock located in the suprachiasmatic nuclei ( SCN ) of the hypothalamus regulates daily temporal organization in behavior and neuroendocrine function .
	manualset3
143978	5	409130	5	NULL	NULL	0	NULL	behavior 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The circadian clock located in the suprachiasmatic nuclei ( SCN ) of the hypothalamus regulates daily temporal organization in behavior and neuroendocrine function .
	manualset3
143979	6	409130	5	NULL	NULL	0	NULL	neuroendocrine function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The circadian clock located in the suprachiasmatic nuclei ( SCN ) of the hypothalamus regulates daily temporal organization in behavior and neuroendocrine function .
	manualset3
143980	1	409131	5	NULL	NULL	0	NULL	circadian typology 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The circadian typology is an individual difference that presented significant relationships with the sleep beliefs , the possibility of the evening-type being a risk factor for a worse sleep hygiene , and the maintenance of sleep problems such as insomnia may all be investigated in depth in future research .
	manualset3
143981	2	409131	5	NULL	NULL	0	NULL	individual difference 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The circadian typology is an individual difference that presented significant relationships with the sleep beliefs , the possibility of the evening-type being a risk factor for a worse sleep hygiene , and the maintenance of sleep problems such as insomnia may all be investigated in depth in future research .
	manualset3
143982	3	409131	5	NULL	NULL	0	NULL	relationships 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The circadian typology is an individual difference that presented significant relationships with the sleep beliefs , the possibility of the evening-type being a risk factor for a worse sleep hygiene , and the maintenance of sleep problems such as insomnia may all be investigated in depth in future research .
	manualset3
143983	4	409131	5	NULL	NULL	0	NULL	sleep beliefs	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The circadian typology is an individual difference that presented significant relationships with the sleep beliefs , the possibility of the evening-type being a risk factor for a worse sleep hygiene , and the maintenance of sleep problems such as insomnia may all be investigated in depth in future research .
	manualset3
143984	5	409131	5	NULL	NULL	0	NULL	possibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The circadian typology is an individual difference that presented significant relationships with the sleep beliefs , the possibility of the evening-type being a risk factor for a worse sleep hygiene , and the maintenance of sleep problems such as insomnia may all be investigated in depth in future research .
	manualset3
143985	6	409131	5	NULL	NULL	0	NULL	evening-type	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The circadian typology is an individual difference that presented significant relationships with the sleep beliefs , the possibility of the evening-type being a risk factor for a worse sleep hygiene , and the maintenance of sleep problems such as insomnia may all be investigated in depth in future research .
	manualset3
143986	7	409131	5	NULL	NULL	0	NULL	risk factor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The circadian typology is an individual difference that presented significant relationships with the sleep beliefs , the possibility of the evening-type being a risk factor for a worse sleep hygiene , and the maintenance of sleep problems such as insomnia may all be investigated in depth in future research .
	manualset3
143987	8	409131	5	NULL	NULL	0	NULL	worse sleep hygiene	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The circadian typology is an individual difference that presented significant relationships with the sleep beliefs , the possibility of the evening-type being a risk factor for a worse sleep hygiene , and the maintenance of sleep problems such as insomnia may all be investigated in depth in future research .
	manualset3
143988	9	409131	5	NULL	NULL	0	NULL	maintenance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The circadian typology is an individual difference that presented significant relationships with the sleep beliefs , the possibility of the evening-type being a risk factor for a worse sleep hygiene , and the maintenance of sleep problems such as insomnia may all be investigated in depth in future research .
	manualset3
143989	10	409131	5	NULL	NULL	0	NULL	sleep problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The circadian typology is an individual difference that presented significant relationships with the sleep beliefs , the possibility of the evening-type being a risk factor for a worse sleep hygiene , and the maintenance of sleep problems such as insomnia may all be investigated in depth in future research .
	manualset3
143990	11	409131	5	NULL	NULL	0	NULL	insomnia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The circadian typology is an individual difference that presented significant relationships with the sleep beliefs , the possibility of the evening-type being a risk factor for a worse sleep hygiene , and the maintenance of sleep problems such as insomnia may all be investigated in depth in future research .
	manualset3
143991	12	409131	5	NULL	NULL	0	NULL	future research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The circadian typology is an individual difference that presented significant relationships with the sleep beliefs , the possibility of the evening-type being a risk factor for a worse sleep hygiene , and the maintenance of sleep problems such as insomnia may all be investigated in depth in future research .
	manualset3
143992	1	409132	5	NULL	NULL	0	NULL	stratification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The city 's stratification according to living conditions and incidence of TB allowed for the identification of risk areas , providing input for the local TB Control Program .
	manualset3
143993	2	409132	5	NULL	NULL	0	NULL	living conditions	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The city 's stratification according to living conditions and incidence of TB allowed for the identification of risk areas , providing input for the local TB Control Program .
	manualset3
143994	3	409132	5	NULL	NULL	0	NULL	incidence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The city 's stratification according to living conditions and incidence of TB allowed for the identification of risk areas , providing input for the local TB Control Program .
	manualset3
143995	4	409132	5	NULL	NULL	0	NULL	TB 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The city 's stratification according to living conditions and incidence of TB allowed for the identification of risk areas , providing input for the local TB Control Program .
	manualset3
143996	5	409132	5	NULL	NULL	0	NULL	identification 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The city 's stratification according to living conditions and incidence of TB allowed for the identification of risk areas , providing input for the local TB Control Program .
	manualset3
143997	6	409132	5	NULL	NULL	0	NULL	risk areas	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The city 's stratification according to living conditions and incidence of TB allowed for the identification of risk areas , providing input for the local TB Control Program .
	manualset3
143998	7	409132	5	NULL	NULL	0	NULL	input 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The city 's stratification according to living conditions and incidence of TB allowed for the identification of risk areas , providing input for the local TB Control Program .
	manualset3
143999	8	409132	5	NULL	NULL	0	NULL	local TB Control Program 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The city 's stratification according to living conditions and incidence of TB allowed for the identification of risk areas , providing input for the local TB Control Program .
	manualset3
144000	1	409133	5	NULL	NULL	0	NULL	short , highly active photoreceptor-specific enhancer/promoter region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A short , highly active photoreceptor-specific enhancer/promoter region upstream of the human rhodopsin kinase gene .
	manualset3
144001	2	409133	5	NULL	NULL	0	NULL	human rhodopsin kinase gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A short , highly active photoreceptor-specific enhancer/promoter region upstream of the human rhodopsin kinase gene .
	manualset3
144002	1	409134	5	NULL	NULL	0	NULL	extension 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The civil work of the extension is already finished and the installation of the equipment has started .
	manualset3
144003	2	409134	5	NULL	NULL	0	NULL	installation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The civil work of the extension is already finished and the installation of the equipment has started .
	manualset3
144004	3	409134	5	NULL	NULL	0	NULL	equipment 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The civil work of the extension is already finished and the installation of the equipment has started .
	manualset3
144005	1	409135	5	NULL	NULL	0	NULL	classification 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The classification of autism , Asperger 's syndrome , and pervasive developmental disorder .
	manualset3
144006	2	409135	5	NULL	NULL	0	NULL	autism 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The classification of autism , Asperger 's syndrome , and pervasive developmental disorder .
	manualset3
144007	3	409135	5	NULL	NULL	0	NULL	Asperger 's syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The classification of autism , Asperger 's syndrome , and pervasive developmental disorder .
	manualset3
144008	4	409135	5	NULL	NULL	0	NULL	pervasive developmental disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The classification of autism , Asperger 's syndrome , and pervasive developmental disorder .
	manualset3
144009	1	409136	5	NULL	NULL	0	NULL	classification 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The classification of vascular lesions of childhood is presented .
	manualset3
144010	2	409136	5	NULL	NULL	0	NULL	vascular lesions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The classification of vascular lesions of childhood is presented .
	manualset3
144011	3	409136	5	NULL	NULL	0	NULL	childhood 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The classification of vascular lesions of childhood is presented .
	manualset3
144012	1	409137	5	NULL	NULL	0	NULL	cleavage 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cleavage of CXCR1 , the functional consequences of its cleavage , and the identification of soluble CXCR1 fragments that behave as bioactive components represent a new pathophysiologic mechanism in cystic fibrosis and other chronic lung diseases .
	manualset3
144013	2	409137	5	NULL	NULL	0	NULL	CXCR1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The cleavage of CXCR1 , the functional consequences of its cleavage , and the identification of soluble CXCR1 fragments that behave as bioactive components represent a new pathophysiologic mechanism in cystic fibrosis and other chronic lung diseases .
	manualset3
144014	3	409137	5	NULL	NULL	0	NULL	functional consequences	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cleavage of CXCR1 , the functional consequences of its cleavage , and the identification of soluble CXCR1 fragments that behave as bioactive components represent a new pathophysiologic mechanism in cystic fibrosis and other chronic lung diseases .
	manualset3
144015	4	409137	5	NULL	NULL	0	NULL	cleavage 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cleavage of CXCR1 , the functional consequences of its cleavage , and the identification of soluble CXCR1 fragments that behave as bioactive components represent a new pathophysiologic mechanism in cystic fibrosis and other chronic lung diseases .
	manualset3
144016	5	409137	5	NULL	NULL	0	NULL	identification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cleavage of CXCR1 , the functional consequences of its cleavage , and the identification of soluble CXCR1 fragments that behave as bioactive components represent a new pathophysiologic mechanism in cystic fibrosis and other chronic lung diseases .
	manualset3
144017	6	409137	5	NULL	NULL	0	NULL	soluble CXCR1 fragments	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The cleavage of CXCR1 , the functional consequences of its cleavage , and the identification of soluble CXCR1 fragments that behave as bioactive components represent a new pathophysiologic mechanism in cystic fibrosis and other chronic lung diseases .
	manualset3
144018	7	409137	5	NULL	NULL	0	NULL	bioactive components	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cleavage of CXCR1 , the functional consequences of its cleavage , and the identification of soluble CXCR1 fragments that behave as bioactive components represent a new pathophysiologic mechanism in cystic fibrosis and other chronic lung diseases .
	manualset3
144019	8	409137	5	NULL	NULL	0	NULL	pathophysiologic mechanism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cleavage of CXCR1 , the functional consequences of its cleavage , and the identification of soluble CXCR1 fragments that behave as bioactive components represent a new pathophysiologic mechanism in cystic fibrosis and other chronic lung diseases .
	manualset3
144020	9	409137	5	NULL	NULL	0	NULL	cystic fibrosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The cleavage of CXCR1 , the functional consequences of its cleavage , and the identification of soluble CXCR1 fragments that behave as bioactive components represent a new pathophysiologic mechanism in cystic fibrosis and other chronic lung diseases .
	manualset3
144021	10	409137	5	NULL	NULL	0	NULL	chronic lung diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The cleavage of CXCR1 , the functional consequences of its cleavage , and the identification of soluble CXCR1 fragments that behave as bioactive components represent a new pathophysiologic mechanism in cystic fibrosis and other chronic lung diseases .
	manualset3
144022	1	409138	5	NULL	NULL	0	NULL	cleavage products 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The cleavage products can act as hormones , signaling compounds , chromophores and scent/aroma constituents .
	manualset3
144023	2	409138	5	NULL	NULL	0	NULL	hormones 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cleavage products can act as hormones , signaling compounds , chromophores and scent/aroma constituents .
	manualset3
144024	3	409138	5	NULL	NULL	0	NULL	signaling compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The cleavage products can act as hormones , signaling compounds , chromophores and scent/aroma constituents .
	manualset3
144025	4	409138	5	NULL	NULL	0	NULL	chromophores 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The cleavage products can act as hormones , signaling compounds , chromophores and scent/aroma constituents .
	manualset3
144026	5	409138	5	NULL	NULL	0	NULL	scent/aroma constituents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The cleavage products can act as hormones , signaling compounds , chromophores and scent/aroma constituents .
	manualset3
144027	1	409139	5	NULL	NULL	0	NULL	cleavage 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cleavage takes place between a cytosine and an adenine moiety , within a possible loop and stem structure ; the cut is in the border between the double-stranded and single-stranded regions of this structure .
	manualset3
144028	2	409139	5	NULL	NULL	NULL	NULL	cytosine 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The cleavage takes place between a cytosine and an adenine moiety , within a possible loop and stem structure ; the cut is in the border between the double-stranded and single-stranded regions of this structure .
	manualset3
144029	3	409139	5	NULL	NULL	NULL	NULL	adenine moiety	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The cleavage takes place between a cytosine and an adenine moiety , within a possible loop and stem structure ; the cut is in the border between the double-stranded and single-stranded regions of this structure .
	manualset3
144030	4	409139	5	NULL	NULL	0	NULL	loop 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cleavage takes place between a cytosine and an adenine moiety , within a possible loop and stem structure ; the cut is in the border between the double-stranded and single-stranded regions of this structure .
	manualset3
144031	5	409139	5	NULL	NULL	0	NULL	stem structure 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cleavage takes place between a cytosine and an adenine moiety , within a possible loop and stem structure ; the cut is in the border between the double-stranded and single-stranded regions of this structure .
	manualset3
144032	6	409139	5	NULL	NULL	0	NULL	cut 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cleavage takes place between a cytosine and an adenine moiety , within a possible loop and stem structure ; the cut is in the border between the double-stranded and single-stranded regions of this structure .
	manualset3
144033	7	409139	5	NULL	NULL	0	NULL	border 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cleavage takes place between a cytosine and an adenine moiety , within a possible loop and stem structure ; the cut is in the border between the double-stranded and single-stranded regions of this structure .
	manualset3
144034	8	409139	5	NULL	NULL	NULL	NULL	double-stranded regions 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The cleavage takes place between a cytosine and an adenine moiety , within a possible loop and stem structure ; the cut is in the border between the double-stranded and single-stranded regions of this structure .
	manualset3
144035	9	409139	5	NULL	NULL	0	NULL	single-stranded regions 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The cleavage takes place between a cytosine and an adenine moiety , within a possible loop and stem structure ; the cut is in the border between the double-stranded and single-stranded regions of this structure .
	manualset3
144036	10	409139	5	NULL	NULL	0	NULL	structure 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cleavage takes place between a cytosine and an adenine moiety , within a possible loop and stem structure ; the cut is in the border between the double-stranded and single-stranded regions of this structure .
	manualset3
144037	1	409140	5	NULL	NULL	0	NULL	cleft indices	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cleft indices and cleft area indices in rat tumor capillaries were significantly higher than in normal brain capillaries , and BK infusion did not alter these indices .
	manualset3
144038	2	409140	5	NULL	NULL	0	NULL	cleft area indices	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cleft indices and cleft area indices in rat tumor capillaries were significantly higher than in normal brain capillaries , and BK infusion did not alter these indices .
	manualset3
144039	3	409140	5	NULL	NULL	0	NULL	rat tumor capillaries 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The cleft indices and cleft area indices in rat tumor capillaries were significantly higher than in normal brain capillaries , and BK infusion did not alter these indices .
	manualset3
144040	4	409140	5	NULL	NULL	0	NULL	normal brain capillaries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The cleft indices and cleft area indices in rat tumor capillaries were significantly higher than in normal brain capillaries , and BK infusion did not alter these indices .
	manualset3
144041	5	409140	5	NULL	NULL	0	NULL	BK infusion 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cleft indices and cleft area indices in rat tumor capillaries were significantly higher than in normal brain capillaries , and BK infusion did not alter these indices .
	manualset3
144042	6	409140	5	NULL	NULL	0	NULL	indices 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cleft indices and cleft area indices in rat tumor capillaries were significantly higher than in normal brain capillaries , and BK infusion did not alter these indices .
	manualset3
144043	1	409141	5	NULL	NULL	0	NULL	short cut	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A short cut to establish hyperhomocysteinemia as a risk factor for arteriosclerosis ?
	manualset3
144044	2	409141	5	NULL	NULL	0	NULL	hyperhomocysteinemia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A short cut to establish hyperhomocysteinemia as a risk factor for arteriosclerosis ?
	manualset3
144045	3	409141	5	NULL	NULL	0	NULL	risk factor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A short cut to establish hyperhomocysteinemia as a risk factor for arteriosclerosis ?
	manualset3
144046	4	409141	5	NULL	NULL	0	NULL	arteriosclerosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A short cut to establish hyperhomocysteinemia as a risk factor for arteriosclerosis ?
	manualset3
144047	1	409142	5	NULL	NULL	0	NULL	clinical manifestations 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical , pathological and radiological manifestations of type 1 Gaucher disease and the role of imaging techniques such as CT , MRI and sulfur-colloid scintigraphy in the management of these patients is discussed .
	manualset3
144048	2	409142	5	NULL	NULL	0	NULL	pathological manifestations 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical , pathological and radiological manifestations of type 1 Gaucher disease and the role of imaging techniques such as CT , MRI and sulfur-colloid scintigraphy in the management of these patients is discussed .
	manualset3
144049	3	409142	5	NULL	NULL	0	NULL	radiological manifestations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical , pathological and radiological manifestations of type 1 Gaucher disease and the role of imaging techniques such as CT , MRI and sulfur-colloid scintigraphy in the management of these patients is discussed .
	manualset3
144050	4	409142	5	NULL	NULL	0	NULL	 type 1 Gaucher disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical , pathological and radiological manifestations of type 1 Gaucher disease and the role of imaging techniques such as CT , MRI and sulfur-colloid scintigraphy in the management of these patients is discussed .
	manualset3
144051	5	409142	5	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical , pathological and radiological manifestations of type 1 Gaucher disease and the role of imaging techniques such as CT , MRI and sulfur-colloid scintigraphy in the management of these patients is discussed .
	manualset3
144052	6	409142	5	NULL	NULL	0	NULL	imaging techniques	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical , pathological and radiological manifestations of type 1 Gaucher disease and the role of imaging techniques such as CT , MRI and sulfur-colloid scintigraphy in the management of these patients is discussed .
	manualset3
144053	7	409142	5	NULL	NULL	0	NULL	CT 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical , pathological and radiological manifestations of type 1 Gaucher disease and the role of imaging techniques such as CT , MRI and sulfur-colloid scintigraphy in the management of these patients is discussed .
	manualset3
144054	8	409142	5	NULL	NULL	0	NULL	MRI 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical , pathological and radiological manifestations of type 1 Gaucher disease and the role of imaging techniques such as CT , MRI and sulfur-colloid scintigraphy in the management of these patients is discussed .
	manualset3
144055	9	409142	5	NULL	NULL	0	NULL	sulfur-colloid scintigraphy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical , pathological and radiological manifestations of type 1 Gaucher disease and the role of imaging techniques such as CT , MRI and sulfur-colloid scintigraphy in the management of these patients is discussed .
	manualset3
144056	10	409142	5	NULL	NULL	0	NULL	management 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical , pathological and radiological manifestations of type 1 Gaucher disease and the role of imaging techniques such as CT , MRI and sulfur-colloid scintigraphy in the management of these patients is discussed .
	manualset3
144057	11	409142	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical , pathological and radiological manifestations of type 1 Gaucher disease and the role of imaging techniques such as CT , MRI and sulfur-colloid scintigraphy in the management of these patients is discussed .
	manualset3
144058	1	409143	5	NULL	NULL	NULL	NULL	clinical assessment file	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The clinical assessment file on tramadol is of low quality .
	manualset3
144059	2	409143	5	NULL	NULL	0	NULL	tramadol 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical assessment file on tramadol is of low quality .
	manualset3
144060	3	409143	5	NULL	NULL	0	NULL	low quality	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical assessment file on tramadol is of low quality .
	manualset3
144061	1	409144	5	NULL	NULL	0	NULL	clinical benefits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical benefits of curcumin as a single agent were demonstrated in patients with advanced pancreatic cancer in a phase 2 study despite pharmacokinetic analysis showing a much lower plasma concentration of curcumin in humans than in vitro .
	manualset3
144062	2	409144	5	NULL	NULL	0	NULL	curcumin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical benefits of curcumin as a single agent were demonstrated in patients with advanced pancreatic cancer in a phase 2 study despite pharmacokinetic analysis showing a much lower plasma concentration of curcumin in humans than in vitro .
	manualset3
144063	3	409144	5	NULL	NULL	0	NULL	single agent 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical benefits of curcumin as a single agent were demonstrated in patients with advanced pancreatic cancer in a phase 2 study despite pharmacokinetic analysis showing a much lower plasma concentration of curcumin in humans than in vitro .
	manualset3
144064	4	409144	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical benefits of curcumin as a single agent were demonstrated in patients with advanced pancreatic cancer in a phase 2 study despite pharmacokinetic analysis showing a much lower plasma concentration of curcumin in humans than in vitro .
	manualset3
144065	5	409144	5	NULL	NULL	0	NULL	advanced pancreatic cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical benefits of curcumin as a single agent were demonstrated in patients with advanced pancreatic cancer in a phase 2 study despite pharmacokinetic analysis showing a much lower plasma concentration of curcumin in humans than in vitro .
	manualset3
144066	6	409144	5	NULL	NULL	0	NULL	phase 2 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical benefits of curcumin as a single agent were demonstrated in patients with advanced pancreatic cancer in a phase 2 study despite pharmacokinetic analysis showing a much lower plasma concentration of curcumin in humans than in vitro .
	manualset3
144067	7	409144	5	NULL	NULL	0	NULL	pharmacokinetic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical benefits of curcumin as a single agent were demonstrated in patients with advanced pancreatic cancer in a phase 2 study despite pharmacokinetic analysis showing a much lower plasma concentration of curcumin in humans than in vitro .
	manualset3
144068	8	409144	5	NULL	NULL	0	NULL	plasma concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical benefits of curcumin as a single agent were demonstrated in patients with advanced pancreatic cancer in a phase 2 study despite pharmacokinetic analysis showing a much lower plasma concentration of curcumin in humans than in vitro .
	manualset3
144069	9	409144	5	NULL	NULL	0	NULL	curcumin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical benefits of curcumin as a single agent were demonstrated in patients with advanced pancreatic cancer in a phase 2 study despite pharmacokinetic analysis showing a much lower plasma concentration of curcumin in humans than in vitro .
	manualset3
144070	10	409144	5	NULL	NULL	0	NULL	humans 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical benefits of curcumin as a single agent were demonstrated in patients with advanced pancreatic cancer in a phase 2 study despite pharmacokinetic analysis showing a much lower plasma concentration of curcumin in humans than in vitro .
	manualset3
144071	1	409145	5	NULL	NULL	0	NULL	clinical biochemical investigation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical biochemical investigation on the malignant bone tumor .
	manualset3
144072	2	409145	5	NULL	NULL	0	NULL	malignant bone tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical biochemical investigation on the malignant bone tumor .
	manualset3
144073	1	409146	5	NULL	NULL	NULL	NULL	clinical course	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The clinical course of acute radiation syndrome depends on the absorbed radiation dose and its distribution .
	manualset3
144074	2	409146	5	NULL	NULL	0	NULL	acute radiation syndrome 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical course of acute radiation syndrome depends on the absorbed radiation dose and its distribution .
	manualset3
144075	3	409146	5	NULL	NULL	0	NULL	absorbed radiation dose 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical course of acute radiation syndrome depends on the absorbed radiation dose and its distribution .
	manualset3
144076	4	409146	5	NULL	NULL	0	NULL	distribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical course of acute radiation syndrome depends on the absorbed radiation dose and its distribution .
	manualset3
144077	1	409147	5	NULL	NULL	NULL	NULL	clinical course 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The clinical course of spontaneous pneumococcus pneumonia in monkeys was characterized by sudden onset , high sustained temperature , leucocytosis , rapid respiration with expiratory grunt , cough , physical signs of consolidation , invasion of the blood by pneurnococci , and termination in death or recovery by crisis about the 7th to 9th day .
	manualset3
144078	2	409147	5	NULL	NULL	0	NULL	spontaneous pneumococcus pneumonia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical course of spontaneous pneumococcus pneumonia in monkeys was characterized by sudden onset , high sustained temperature , leucocytosis , rapid respiration with expiratory grunt , cough , physical signs of consolidation , invasion of the blood by pneurnococci , and termination in death or recovery by crisis about the 7th to 9th day .
	manualset3
144079	3	409147	5	NULL	NULL	0	NULL	monkeys 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical course of spontaneous pneumococcus pneumonia in monkeys was characterized by sudden onset , high sustained temperature , leucocytosis , rapid respiration with expiratory grunt , cough , physical signs of consolidation , invasion of the blood by pneurnococci , and termination in death or recovery by crisis about the 7th to 9th day .
	manualset3
144080	4	409147	5	NULL	NULL	0	NULL	sudden onset 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical course of spontaneous pneumococcus pneumonia in monkeys was characterized by sudden onset , high sustained temperature , leucocytosis , rapid respiration with expiratory grunt , cough , physical signs of consolidation , invasion of the blood by pneurnococci , and termination in death or recovery by crisis about the 7th to 9th day .
	manualset3
144081	5	409147	5	NULL	NULL	0	NULL	high sustained temperature	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical course of spontaneous pneumococcus pneumonia in monkeys was characterized by sudden onset , high sustained temperature , leucocytosis , rapid respiration with expiratory grunt , cough , physical signs of consolidation , invasion of the blood by pneurnococci , and termination in death or recovery by crisis about the 7th to 9th day .
	manualset3
144082	6	409147	5	NULL	NULL	0	NULL	leucocytosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical course of spontaneous pneumococcus pneumonia in monkeys was characterized by sudden onset , high sustained temperature , leucocytosis , rapid respiration with expiratory grunt , cough , physical signs of consolidation , invasion of the blood by pneurnococci , and termination in death or recovery by crisis about the 7th to 9th day .
	manualset3
144083	7	409147	5	NULL	NULL	0	NULL	rapid respiration with expiratory grunt	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical course of spontaneous pneumococcus pneumonia in monkeys was characterized by sudden onset , high sustained temperature , leucocytosis , rapid respiration with expiratory grunt , cough , physical signs of consolidation , invasion of the blood by pneurnococci , and termination in death or recovery by crisis about the 7th to 9th day .
	manualset3
144084	8	409147	5	NULL	NULL	0	NULL	cough 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical course of spontaneous pneumococcus pneumonia in monkeys was characterized by sudden onset , high sustained temperature , leucocytosis , rapid respiration with expiratory grunt , cough , physical signs of consolidation , invasion of the blood by pneurnococci , and termination in death or recovery by crisis about the 7th to 9th day .
	manualset3
144085	9	409147	5	NULL	NULL	0	NULL	physical signs of consolidation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical course of spontaneous pneumococcus pneumonia in monkeys was characterized by sudden onset , high sustained temperature , leucocytosis , rapid respiration with expiratory grunt , cough , physical signs of consolidation , invasion of the blood by pneurnococci , and termination in death or recovery by crisis about the 7th to 9th day .
	manualset3
144086	10	409147	5	NULL	NULL	0	NULL	invasion of the blood by pneurnococci 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical course of spontaneous pneumococcus pneumonia in monkeys was characterized by sudden onset , high sustained temperature , leucocytosis , rapid respiration with expiratory grunt , cough , physical signs of consolidation , invasion of the blood by pneurnococci , and termination in death or recovery by crisis about the 7th to 9th day .
	manualset3
144087	11	409147	5	NULL	NULL	0	NULL	termination 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical course of spontaneous pneumococcus pneumonia in monkeys was characterized by sudden onset , high sustained temperature , leucocytosis , rapid respiration with expiratory grunt , cough , physical signs of consolidation , invasion of the blood by pneurnococci , and termination in death or recovery by crisis about the 7th to 9th day .
	manualset3
144088	12	409147	5	NULL	NULL	0	NULL	death 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical course of spontaneous pneumococcus pneumonia in monkeys was characterized by sudden onset , high sustained temperature , leucocytosis , rapid respiration with expiratory grunt , cough , physical signs of consolidation , invasion of the blood by pneurnococci , and termination in death or recovery by crisis about the 7th to 9th day .
	manualset3
144089	13	409147	5	NULL	NULL	0	NULL	recovery 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical course of spontaneous pneumococcus pneumonia in monkeys was characterized by sudden onset , high sustained temperature , leucocytosis , rapid respiration with expiratory grunt , cough , physical signs of consolidation , invasion of the blood by pneurnococci , and termination in death or recovery by crisis about the 7th to 9th day .
	manualset3
144090	14	409147	5	NULL	NULL	0	NULL	crisis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical course of spontaneous pneumococcus pneumonia in monkeys was characterized by sudden onset , high sustained temperature , leucocytosis , rapid respiration with expiratory grunt , cough , physical signs of consolidation , invasion of the blood by pneurnococci , and termination in death or recovery by crisis about the 7th to 9th day .
	manualset3
144091	15	409147	5	NULL	NULL	0	NULL	7th to 9th day	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical course of spontaneous pneumococcus pneumonia in monkeys was characterized by sudden onset , high sustained temperature , leucocytosis , rapid respiration with expiratory grunt , cough , physical signs of consolidation , invasion of the blood by pneurnococci , and termination in death or recovery by crisis about the 7th to 9th day .
	manualset3
144092	1	409148	5	NULL	NULL	0	NULL	clinical course	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical course was characterized by urinary symptoms and by presence the cysts in urine .
	manualset3
144093	2	409148	5	NULL	NULL	0	NULL	urinary symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical course was characterized by urinary symptoms and by presence the cysts in urine .
	manualset3
144094	3	409148	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical course was characterized by urinary symptoms and by presence the cysts in urine .
	manualset3
144095	4	409148	5	NULL	NULL	0	NULL	cysts 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical course was characterized by urinary symptoms and by presence the cysts in urine .
	manualset3
144096	5	409148	5	NULL	NULL	0	NULL	urine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical course was characterized by urinary symptoms and by presence the cysts in urine .
	manualset3
144097	1	409149	5	NULL	NULL	0	NULL	clinical diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical diagnosis of abnormal hand tremor correlated well with the presence of motor unit entrainment in the forearm EMG and with writing or drawing tremor that was measurable with a digitizing tablet .
	manualset3
144098	2	409149	5	NULL	NULL	0	NULL	abnormal hand tremor 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical diagnosis of abnormal hand tremor correlated well with the presence of motor unit entrainment in the forearm EMG and with writing or drawing tremor that was measurable with a digitizing tablet .
	manualset3
144099	3	409149	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical diagnosis of abnormal hand tremor correlated well with the presence of motor unit entrainment in the forearm EMG and with writing or drawing tremor that was measurable with a digitizing tablet .
	manualset3
144100	4	409149	5	NULL	NULL	0	NULL	motor unit entrainment	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical diagnosis of abnormal hand tremor correlated well with the presence of motor unit entrainment in the forearm EMG and with writing or drawing tremor that was measurable with a digitizing tablet .
	manualset3
144101	5	409149	5	NULL	NULL	0	NULL	forearm EMG	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical diagnosis of abnormal hand tremor correlated well with the presence of motor unit entrainment in the forearm EMG and with writing or drawing tremor that was measurable with a digitizing tablet .
	manualset3
144102	6	409149	5	NULL	NULL	0	NULL	writing tremor 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical diagnosis of abnormal hand tremor correlated well with the presence of motor unit entrainment in the forearm EMG and with writing or drawing tremor that was measurable with a digitizing tablet .
	manualset3
144103	7	409149	5	NULL	NULL	0	NULL	drawing tremor 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical diagnosis of abnormal hand tremor correlated well with the presence of motor unit entrainment in the forearm EMG and with writing or drawing tremor that was measurable with a digitizing tablet .
	manualset3
144104	8	409149	5	NULL	NULL	0	NULL	digitizing tablet 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical diagnosis of abnormal hand tremor correlated well with the presence of motor unit entrainment in the forearm EMG and with writing or drawing tremor that was measurable with a digitizing tablet .
	manualset3
144105	1	409150	5	NULL	NULL	0	NULL	clinical effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical effect for 87 cases of acute simple cystitis was excellent in 54 cases ( 62 % ) , moderate in 24 cases ( 27.6 % ) and poor 9 cases ( 10.3 % ) , overall effective rate being 89.7 % .
	manualset3
144106	2	409150	5	NULL	NULL	0	NULL	87 cases	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical effect for 87 cases of acute simple cystitis was excellent in 54 cases ( 62 % ) , moderate in 24 cases ( 27.6 % ) and poor 9 cases ( 10.3 % ) , overall effective rate being 89.7 % .
	manualset3
144107	3	409150	5	NULL	NULL	0	NULL	acute simple cystitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical effect for 87 cases of acute simple cystitis was excellent in 54 cases ( 62 % ) , moderate in 24 cases ( 27.6 % ) and poor 9 cases ( 10.3 % ) , overall effective rate being 89.7 % .
	manualset3
144108	4	409150	5	NULL	NULL	0	NULL	54 cases ( 62 % ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical effect for 87 cases of acute simple cystitis was excellent in 54 cases ( 62 % ) , moderate in 24 cases ( 27.6 % ) and poor 9 cases ( 10.3 % ) , overall effective rate being 89.7 % .
	manualset3
144109	5	409150	5	NULL	NULL	0	NULL	24 cases ( 27.6 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical effect for 87 cases of acute simple cystitis was excellent in 54 cases ( 62 % ) , moderate in 24 cases ( 27.6 % ) and poor 9 cases ( 10.3 % ) , overall effective rate being 89.7 % .
	manualset3
144110	6	409150	5	NULL	NULL	0	NULL	9 cases ( 10.3 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical effect for 87 cases of acute simple cystitis was excellent in 54 cases ( 62 % ) , moderate in 24 cases ( 27.6 % ) and poor 9 cases ( 10.3 % ) , overall effective rate being 89.7 % .
	manualset3
144111	7	409150	5	NULL	NULL	0	NULL	effective rate 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical effect for 87 cases of acute simple cystitis was excellent in 54 cases ( 62 % ) , moderate in 24 cases ( 27.6 % ) and poor 9 cases ( 10.3 % ) , overall effective rate being 89.7 % .
	manualset3
144112	8	409150	5	NULL	NULL	0	NULL	89.7 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical effect for 87 cases of acute simple cystitis was excellent in 54 cases ( 62 % ) , moderate in 24 cases ( 27.6 % ) and poor 9 cases ( 10.3 % ) , overall effective rate being 89.7 % .
	manualset3
144113	1	409151	5	NULL	NULL	0	NULL	clinical implications 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical implications of the results of exercise tests in asthmatics , their relatives , and other subjects are considered in terms of the diagnosis and prognosis of asthma and its mode of inheritance .
	manualset3
144114	2	409151	5	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical implications of the results of exercise tests in asthmatics , their relatives , and other subjects are considered in terms of the diagnosis and prognosis of asthma and its mode of inheritance .
	manualset3
144115	3	409151	5	NULL	NULL	0	NULL	exercise tests	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical implications of the results of exercise tests in asthmatics , their relatives , and other subjects are considered in terms of the diagnosis and prognosis of asthma and its mode of inheritance .
	manualset3
144116	4	409151	5	NULL	NULL	0	NULL	asthmatics 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical implications of the results of exercise tests in asthmatics , their relatives , and other subjects are considered in terms of the diagnosis and prognosis of asthma and its mode of inheritance .
	manualset3
144117	5	409151	5	NULL	NULL	0	NULL	relatives 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical implications of the results of exercise tests in asthmatics , their relatives , and other subjects are considered in terms of the diagnosis and prognosis of asthma and its mode of inheritance .
	manualset3
144118	6	409151	5	NULL	NULL	0	NULL	subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical implications of the results of exercise tests in asthmatics , their relatives , and other subjects are considered in terms of the diagnosis and prognosis of asthma and its mode of inheritance .
	manualset3
144119	7	409151	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical implications of the results of exercise tests in asthmatics , their relatives , and other subjects are considered in terms of the diagnosis and prognosis of asthma and its mode of inheritance .
	manualset3
144120	8	409151	5	NULL	NULL	0	NULL	prognosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical implications of the results of exercise tests in asthmatics , their relatives , and other subjects are considered in terms of the diagnosis and prognosis of asthma and its mode of inheritance .
	manualset3
144121	9	409151	5	NULL	NULL	0	NULL	asthma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical implications of the results of exercise tests in asthmatics , their relatives , and other subjects are considered in terms of the diagnosis and prognosis of asthma and its mode of inheritance .
	manualset3
144122	10	409151	5	NULL	NULL	0	NULL	mode of inheritance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical implications of the results of exercise tests in asthmatics , their relatives , and other subjects are considered in terms of the diagnosis and prognosis of asthma and its mode of inheritance .
	manualset3
144123	1	409152	5	NULL	NULL	0	NULL	clinical outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical outcome of granulocyte transfusion therapy is often hampered by short ex vivo shelf life , inefficiency of recruitment to sites of inflammation , and poor pathogen-killing capability of transplanted neutrophils .
	manualset3
144124	2	409152	5	NULL	NULL	0	NULL	granulocyte transfusion therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical outcome of granulocyte transfusion therapy is often hampered by short ex vivo shelf life , inefficiency of recruitment to sites of inflammation , and poor pathogen-killing capability of transplanted neutrophils .
	manualset3
144125	3	409152	5	NULL	NULL	0	NULL	shelf life	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical outcome of granulocyte transfusion therapy is often hampered by short ex vivo shelf life , inefficiency of recruitment to sites of inflammation , and poor pathogen-killing capability of transplanted neutrophils .
	manualset3
144126	4	409152	5	NULL	NULL	0	NULL	inefficiency of recruitment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical outcome of granulocyte transfusion therapy is often hampered by short ex vivo shelf life , inefficiency of recruitment to sites of inflammation , and poor pathogen-killing capability of transplanted neutrophils .
	manualset3
144127	5	409152	5	NULL	NULL	0	NULL	sites of inflammation	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical outcome of granulocyte transfusion therapy is often hampered by short ex vivo shelf life , inefficiency of recruitment to sites of inflammation , and poor pathogen-killing capability of transplanted neutrophils .
	manualset3
144128	6	409152	5	NULL	NULL	0	NULL	poor pathogen-killing capability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical outcome of granulocyte transfusion therapy is often hampered by short ex vivo shelf life , inefficiency of recruitment to sites of inflammation , and poor pathogen-killing capability of transplanted neutrophils .
	manualset3
144129	7	409152	5	NULL	NULL	0	NULL	transplanted neutrophils	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical outcome of granulocyte transfusion therapy is often hampered by short ex vivo shelf life , inefficiency of recruitment to sites of inflammation , and poor pathogen-killing capability of transplanted neutrophils .
	manualset3
144130	1	409153	5	NULL	NULL	0	NULL	clinical outcome 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical outcome of peripheral nerve injuries requiring surgical repair is usually poor and efficient therapies do not exist .
	manualset3
144131	2	409153	5	NULL	NULL	0	NULL	peripheral nerve injuries 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical outcome of peripheral nerve injuries requiring surgical repair is usually poor and efficient therapies do not exist .
	manualset3
144132	3	409153	5	NULL	NULL	0	NULL	surgical repair	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical outcome of peripheral nerve injuries requiring surgical repair is usually poor and efficient therapies do not exist .
	manualset3
144133	4	409153	5	NULL	NULL	0	NULL	therapies 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical outcome of peripheral nerve injuries requiring surgical repair is usually poor and efficient therapies do not exist .
	manualset3
144134	1	409154	5	NULL	NULL	0	NULL	clinical outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical outcomes of patients with MAP reduction ) 20 % following dural opening during surgery were significantly poorer than those of patients without this amount of blood pressure reduction .
	manualset3
144135	2	409154	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical outcomes of patients with MAP reduction ) 20 % following dural opening during surgery were significantly poorer than those of patients without this amount of blood pressure reduction .
	manualset3
144136	3	409154	5	NULL	NULL	0	NULL	MAP reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical outcomes of patients with MAP reduction ) 20 % following dural opening during surgery were significantly poorer than those of patients without this amount of blood pressure reduction .
	manualset3
144137	4	409154	5	NULL	NULL	0	NULL	20 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical outcomes of patients with MAP reduction ) 20 % following dural opening during surgery were significantly poorer than those of patients without this amount of blood pressure reduction .
	manualset3
144138	5	409154	5	NULL	NULL	0	NULL	dural opening	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical outcomes of patients with MAP reduction ) 20 % following dural opening during surgery were significantly poorer than those of patients without this amount of blood pressure reduction .
	manualset3
144139	6	409154	5	NULL	NULL	0	NULL	surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical outcomes of patients with MAP reduction ) 20 % following dural opening during surgery were significantly poorer than those of patients without this amount of blood pressure reduction .
	manualset3
144140	7	409154	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical outcomes of patients with MAP reduction ) 20 % following dural opening during surgery were significantly poorer than those of patients without this amount of blood pressure reduction .
	manualset3
144141	8	409154	5	NULL	NULL	0	NULL	blood pressure reduction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical outcomes of patients with MAP reduction ) 20 % following dural opening during surgery were significantly poorer than those of patients without this amount of blood pressure reduction .
	manualset3
144142	1	409155	5	NULL	NULL	0	NULL	short form of the prolactin ( PRL ) receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A short form of the prolactin ( PRL ) receptor is able to rescue mammopoiesis in heterozygous PRL receptor mice .
	manualset3
144143	2	409155	5	NULL	NULL	0	NULL	mammopoiesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A short form of the prolactin ( PRL ) receptor is able to rescue mammopoiesis in heterozygous PRL receptor mice .
	manualset3
144144	3	409155	5	NULL	NULL	0	NULL	 heterozygous PRL receptor mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A short form of the prolactin ( PRL ) receptor is able to rescue mammopoiesis in heterozygous PRL receptor mice .
	manualset3
144145	1	409156	5	NULL	NULL	0	NULL	clinical presentation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical presentation , diagnosis and management of V-P shunt-related broncho-pleural fistulae are discussed .
	manualset3
144146	2	409156	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical presentation , diagnosis and management of V-P shunt-related broncho-pleural fistulae are discussed .
	manualset3
144147	3	409156	5	NULL	NULL	0	NULL	management 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical presentation , diagnosis and management of V-P shunt-related broncho-pleural fistulae are discussed .
	manualset3
144148	4	409156	5	NULL	NULL	0	NULL	V-P shunt-related broncho-pleural fistulae	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical presentation , diagnosis and management of V-P shunt-related broncho-pleural fistulae are discussed .
	manualset3
144149	1	409157	5	NULL	NULL	0	NULL	clinical relevance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical relevance of coronary anomalies is discussed particularly for the ill-defined group of anomalies that only occasionally cause severe clinical events comprising anomalous origination of a coronary artery from the opposite sinus ( ACAOS ) , coronary artery fistulae and myocardial bridging .
	manualset3
144150	2	409157	5	NULL	NULL	0	NULL	coronary anomalies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical relevance of coronary anomalies is discussed particularly for the ill-defined group of anomalies that only occasionally cause severe clinical events comprising anomalous origination of a coronary artery from the opposite sinus ( ACAOS ) , coronary artery fistulae and myocardial bridging .
	manualset3
144151	3	409157	5	NULL	NULL	0	NULL	ill-defined group of anomalies 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical relevance of coronary anomalies is discussed particularly for the ill-defined group of anomalies that only occasionally cause severe clinical events comprising anomalous origination of a coronary artery from the opposite sinus ( ACAOS ) , coronary artery fistulae and myocardial bridging .
	manualset3
144152	4	409157	5	NULL	NULL	0	NULL	severe clinical events	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical relevance of coronary anomalies is discussed particularly for the ill-defined group of anomalies that only occasionally cause severe clinical events comprising anomalous origination of a coronary artery from the opposite sinus ( ACAOS ) , coronary artery fistulae and myocardial bridging .
	manualset3
144153	5	409157	5	NULL	NULL	NULL	NULL	 anomalous origination of a coronary artery from the opposite sinus ( ACAOS )	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The clinical relevance of coronary anomalies is discussed particularly for the ill-defined group of anomalies that only occasionally cause severe clinical events comprising anomalous origination of a coronary artery from the opposite sinus ( ACAOS ) , coronary artery fistulae and myocardial bridging .
	manualset3
144154	6	409157	5	NULL	NULL	NULL	NULL	coronary artery fistulae	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The clinical relevance of coronary anomalies is discussed particularly for the ill-defined group of anomalies that only occasionally cause severe clinical events comprising anomalous origination of a coronary artery from the opposite sinus ( ACAOS ) , coronary artery fistulae and myocardial bridging .
	manualset3
144155	7	409157	5	NULL	NULL	0	NULL	myocardial bridging	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical relevance of coronary anomalies is discussed particularly for the ill-defined group of anomalies that only occasionally cause severe clinical events comprising anomalous origination of a coronary artery from the opposite sinus ( ACAOS ) , coronary artery fistulae and myocardial bridging .
	manualset3
144156	1	409158	5	NULL	NULL	0	NULL	clinical significance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical significance of pre - and post-ESWL hydronephrosis found by sonography must be considered in conjunction with the patient 's symptoms , laboratory data , and other radiographic studies .
	manualset3
144157	2	409158	5	NULL	NULL	0	NULL	pre-ESWL hydronephrosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical significance of pre - and post-ESWL hydronephrosis found by sonography must be considered in conjunction with the patient 's symptoms , laboratory data , and other radiographic studies .
	manualset3
144158	3	409158	5	NULL	NULL	0	NULL	post-ESWL hydronephrosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical significance of pre - and post-ESWL hydronephrosis found by sonography must be considered in conjunction with the patient 's symptoms , laboratory data , and other radiographic studies .
	manualset3
144159	4	409158	5	NULL	NULL	0	NULL	sonography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical significance of pre - and post-ESWL hydronephrosis found by sonography must be considered in conjunction with the patient 's symptoms , laboratory data , and other radiographic studies .
	manualset3
144160	5	409158	5	NULL	NULL	0	NULL	conjunction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical significance of pre - and post-ESWL hydronephrosis found by sonography must be considered in conjunction with the patient 's symptoms , laboratory data , and other radiographic studies .
	manualset3
144161	6	409158	5	NULL	NULL	0	NULL	 patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical significance of pre - and post-ESWL hydronephrosis found by sonography must be considered in conjunction with the patient 's symptoms , laboratory data , and other radiographic studies .
	manualset3
144162	7	409158	5	NULL	NULL	0	NULL	symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical significance of pre - and post-ESWL hydronephrosis found by sonography must be considered in conjunction with the patient 's symptoms , laboratory data , and other radiographic studies .
	manualset3
144163	8	409158	5	NULL	NULL	0	NULL	laboratory data	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical significance of pre - and post-ESWL hydronephrosis found by sonography must be considered in conjunction with the patient 's symptoms , laboratory data , and other radiographic studies .
	manualset3
144164	9	409158	5	NULL	NULL	0	NULL	radiographic studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical significance of pre - and post-ESWL hydronephrosis found by sonography must be considered in conjunction with the patient 's symptoms , laboratory data , and other radiographic studies .
	manualset3
144165	1	409159	5	NULL	NULL	0	NULL	clinical significance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical significance of reflex changes produced by vibration .
	manualset3
144166	2	409159	5	NULL	NULL	0	NULL	reflex changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical significance of reflex changes produced by vibration .
	manualset3
144167	3	409159	5	NULL	NULL	0	NULL	vibration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical significance of reflex changes produced by vibration .
	manualset3
144168	1	409160	5	NULL	NULL	0	NULL	clinical spectrum	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical spectrum of supraventricular tachyarrhythmias ranges from infrequent , brief and well tolerated episodes of arrhythmia to attacks resulting in cardiovascular collapse .
	manualset3
144169	2	409160	5	NULL	NULL	0	NULL	supraventricular tachyarrhythmias 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical spectrum of supraventricular tachyarrhythmias ranges from infrequent , brief and well tolerated episodes of arrhythmia to attacks resulting in cardiovascular collapse .
	manualset3
144170	3	409160	5	NULL	NULL	NULL	NULL	episodes 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The clinical spectrum of supraventricular tachyarrhythmias ranges from infrequent , brief and well tolerated episodes of arrhythmia to attacks resulting in cardiovascular collapse .
	manualset3
144171	4	409160	5	NULL	NULL	0	NULL	arrhythmia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical spectrum of supraventricular tachyarrhythmias ranges from infrequent , brief and well tolerated episodes of arrhythmia to attacks resulting in cardiovascular collapse .
	manualset3
144172	5	409160	5	NULL	NULL	0	NULL	attacks 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical spectrum of supraventricular tachyarrhythmias ranges from infrequent , brief and well tolerated episodes of arrhythmia to attacks resulting in cardiovascular collapse .
	manualset3
144173	6	409160	5	NULL	NULL	0	NULL	cardiovascular collapse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical spectrum of supraventricular tachyarrhythmias ranges from infrequent , brief and well tolerated episodes of arrhythmia to attacks resulting in cardiovascular collapse .
	manualset3
144174	1	409161	5	NULL	NULL	0	NULL	clinical symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical symptoms are mostly like enteritis , enterocolitis , acute abdomen or ileitis terminalis .
	manualset3
144175	2	409161	5	NULL	NULL	0	NULL	enteritis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical symptoms are mostly like enteritis , enterocolitis , acute abdomen or ileitis terminalis .
	manualset3
144176	3	409161	5	NULL	NULL	0	NULL	enterocolitis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical symptoms are mostly like enteritis , enterocolitis , acute abdomen or ileitis terminalis .
	manualset3
144177	4	409161	5	NULL	NULL	0	NULL	acute abdomen	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical symptoms are mostly like enteritis , enterocolitis , acute abdomen or ileitis terminalis .
	manualset3
144178	5	409161	5	NULL	NULL	0	NULL	ileitis terminalis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical symptoms are mostly like enteritis , enterocolitis , acute abdomen or ileitis terminalis .
	manualset3
144179	1	409162	5	NULL	NULL	0	NULL	Chronic arteriomesenterial compression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Chronic arteriomesenterial compression on the duodenum ) .
	manualset3
144180	2	409162	5	NULL	NULL	0	NULL	duodenum 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Chronic arteriomesenterial compression on the duodenum ) .
	manualset3
144181	1	409163	5	NULL	NULL	0	NULL	clinical usefulness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical usefulness of the method will require future testing , as the technique has not yet been clinically proven .
	manualset3
144182	2	409163	5	NULL	NULL	0	NULL	method 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical usefulness of the method will require future testing , as the technique has not yet been clinically proven .
	manualset3
144183	3	409163	5	NULL	NULL	0	NULL	future 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical usefulness of the method will require future testing , as the technique has not yet been clinically proven .
	manualset3
144184	4	409163	5	NULL	NULL	0	NULL	testing 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical usefulness of the method will require future testing , as the technique has not yet been clinically proven .
	manualset3
144185	5	409163	5	NULL	NULL	0	NULL	technique 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical usefulness of the method will require future testing , as the technique has not yet been clinically proven .
	manualset3
144186	1	409164	5	NULL	NULL	0	NULL	clinicopathological experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinicopathological experience with 50 cases of pineal region tumors at Clinica Puerta de Hierro is presented .
	manualset3
144187	2	409164	5	NULL	NULL	0	NULL	 50 cases 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinicopathological experience with 50 cases of pineal region tumors at Clinica Puerta de Hierro is presented .
	manualset3
144188	3	409164	5	NULL	NULL	0	NULL	pineal region tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinicopathological experience with 50 cases of pineal region tumors at Clinica Puerta de Hierro is presented .
	manualset3
144189	4	409164	5	NULL	NULL	0	NULL	Clinica Puerta de Hierro	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinicopathological experience with 50 cases of pineal region tumors at Clinica Puerta de Hierro is presented .
	manualset3
144190	1	409165	5	NULL	NULL	0	NULL	clock gene Per2	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The clock gene Per2 influences the glutamatergic system and modulates alcohol consumption .
	manualset3
144191	2	409165	5	NULL	NULL	0	NULL	glutamatergic system	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The clock gene Per2 influences the glutamatergic system and modulates alcohol consumption .
	manualset3
144192	3	409165	5	NULL	NULL	0	NULL	alcohol consumption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The clock gene Per2 influences the glutamatergic system and modulates alcohol consumption .
	manualset3
144193	1	409166	5	NULL	NULL	0	NULL	clone 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The clone with the longest insert -- called pHC1 -- was sequenced and used as a probe for Northern blotting .
	manualset3
144194	2	409166	5	NULL	NULL	0	NULL	longest insert	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The clone with the longest insert -- called pHC1 -- was sequenced and used as a probe for Northern blotting .
	manualset3
144195	3	409166	5	NULL	NULL	0	NULL	pHC1	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The clone with the longest insert -- called pHC1 -- was sequenced and used as a probe for Northern blotting .
	manualset3
144196	4	409166	5	NULL	NULL	0	NULL	probe 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The clone with the longest insert -- called pHC1 -- was sequenced and used as a probe for Northern blotting .
	manualset3
144197	5	409166	5	NULL	NULL	0	NULL	Northern blotting	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The clone with the longest insert -- called pHC1 -- was sequenced and used as a probe for Northern blotting .
	manualset3
144198	1	409167	5	NULL	NULL	0	NULL	clones 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The clones exhibited contact-inhibited , anchorage - and growth factor-dependent growth and did not form tumors in nude mice , suggesting that the cells were not transformed .
	manualset3
144199	2	409167	5	NULL	NULL	0	NULL	contact-inhibited , anchorage - and growth factor-dependent growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The clones exhibited contact-inhibited , anchorage - and growth factor-dependent growth and did not form tumors in nude mice , suggesting that the cells were not transformed .
	manualset3
144200	3	409167	5	NULL	NULL	0	NULL	tumors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clones exhibited contact-inhibited , anchorage - and growth factor-dependent growth and did not form tumors in nude mice , suggesting that the cells were not transformed .
	manualset3
144201	4	409167	5	NULL	NULL	0	NULL	nude mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The clones exhibited contact-inhibited , anchorage - and growth factor-dependent growth and did not form tumors in nude mice , suggesting that the cells were not transformed .
	manualset3
144202	5	409167	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The clones exhibited contact-inhibited , anchorage - and growth factor-dependent growth and did not form tumors in nude mice , suggesting that the cells were not transformed .
	manualset3
144203	1	409168	5	NULL	NULL	0	NULL	clones 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The clones possessed pronounced virulence , but showed different heat sensitivity ( T50 + , T50 + / - ) and resistance to the action of urea ( Ur and U + / - ) .
	manualset3
144204	2	409168	5	NULL	NULL	0	NULL	virulence 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The clones possessed pronounced virulence , but showed different heat sensitivity ( T50 + , T50 + / - ) and resistance to the action of urea ( Ur and U + / - ) .
	manualset3
144205	3	409168	5	NULL	NULL	0	NULL	heat sensitivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The clones possessed pronounced virulence , but showed different heat sensitivity ( T50 + , T50 + / - ) and resistance to the action of urea ( Ur and U + / - ) .
	manualset3
144206	4	409168	5	NULL	NULL	0	NULL	 T50 +	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The clones possessed pronounced virulence , but showed different heat sensitivity ( T50 + , T50 + / - ) and resistance to the action of urea ( Ur and U + / - ) .
	manualset3
144207	5	409168	5	NULL	NULL	0	NULL	 T50 + / -	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The clones possessed pronounced virulence , but showed different heat sensitivity ( T50 + , T50 + / - ) and resistance to the action of urea ( Ur and U + / - ) .
	manualset3
144208	6	409168	5	NULL	NULL	0	NULL	resistance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The clones possessed pronounced virulence , but showed different heat sensitivity ( T50 + , T50 + / - ) and resistance to the action of urea ( Ur and U + / - ) .
	manualset3
144209	7	409168	5	NULL	NULL	0	NULL	action 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The clones possessed pronounced virulence , but showed different heat sensitivity ( T50 + , T50 + / - ) and resistance to the action of urea ( Ur and U + / - ) .
	manualset3
144210	8	409168	5	NULL	NULL	0	NULL	urea 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The clones possessed pronounced virulence , but showed different heat sensitivity ( T50 + , T50 + / - ) and resistance to the action of urea ( Ur and U + / - ) .
	manualset3
144211	9	409168	5	NULL	NULL	0	NULL	Ur 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The clones possessed pronounced virulence , but showed different heat sensitivity ( T50 + , T50 + / - ) and resistance to the action of urea ( Ur and U + / - ) .
	manualset3
144212	10	409168	5	NULL	NULL	0	NULL	 U + / -	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The clones possessed pronounced virulence , but showed different heat sensitivity ( T50 + , T50 + / - ) and resistance to the action of urea ( Ur and U + / - ) .
	manualset3
144213	1	409169	5	NULL	NULL	0	NULL	cloning 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cloning and mapping of these genes together with the fine mapping of the three known genes indicates that the transcriptional map of this region is likely to be complete .
	manualset3
144214	2	409169	5	NULL	NULL	0	NULL	mapping 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cloning and mapping of these genes together with the fine mapping of the three known genes indicates that the transcriptional map of this region is likely to be complete .
	manualset3
144215	3	409169	5	NULL	NULL	NULL	NULL	genes 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The cloning and mapping of these genes together with the fine mapping of the three known genes indicates that the transcriptional map of this region is likely to be complete .
	manualset3
144216	4	409169	5	NULL	NULL	0	NULL	fine mapping	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cloning and mapping of these genes together with the fine mapping of the three known genes indicates that the transcriptional map of this region is likely to be complete .
	manualset3
144217	5	409169	5	NULL	NULL	0	NULL	three 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The cloning and mapping of these genes together with the fine mapping of the three known genes indicates that the transcriptional map of this region is likely to be complete .
	manualset3
144218	6	409169	5	NULL	NULL	0	NULL	genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The cloning and mapping of these genes together with the fine mapping of the three known genes indicates that the transcriptional map of this region is likely to be complete .
	manualset3
144219	7	409169	5	NULL	NULL	0	NULL	transcriptional map	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The cloning and mapping of these genes together with the fine mapping of the three known genes indicates that the transcriptional map of this region is likely to be complete .
	manualset3
144220	8	409169	5	NULL	NULL	0	NULL	region 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The cloning and mapping of these genes together with the fine mapping of the three known genes indicates that the transcriptional map of this region is likely to be complete .
	manualset3
144221	1	409170	5	NULL	NULL	0	NULL	cloning 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cloning and sequencing of a gene from Rickettsia rickettsii which confers hemolytic activity on Escherichia coli strain TB1 is described .
	manualset3
144222	2	409170	5	NULL	NULL	0	NULL	sequencing 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cloning and sequencing of a gene from Rickettsia rickettsii which confers hemolytic activity on Escherichia coli strain TB1 is described .
	manualset3
144223	3	409170	5	NULL	NULL	0	NULL	gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The cloning and sequencing of a gene from Rickettsia rickettsii which confers hemolytic activity on Escherichia coli strain TB1 is described .
	manualset3
144224	4	409170	5	NULL	NULL	0	NULL	Rickettsia rickettsii 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The cloning and sequencing of a gene from Rickettsia rickettsii which confers hemolytic activity on Escherichia coli strain TB1 is described .
	manualset3
144225	5	409170	5	NULL	NULL	0	NULL	hemolytic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cloning and sequencing of a gene from Rickettsia rickettsii which confers hemolytic activity on Escherichia coli strain TB1 is described .
	manualset3
144226	6	409170	5	NULL	NULL	0	NULL	Escherichia coli strain TB1	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The cloning and sequencing of a gene from Rickettsia rickettsii which confers hemolytic activity on Escherichia coli strain TB1 is described .
	manualset3
144227	1	409171	5	NULL	NULL	0	NULL	inhibitory effect 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A showed the strongest inhibitory effect on HO-8910 ( IC50 = 21 microg/ml ) and Bel-7402 cells ( 16 mcirog/ml ) , whereas Fr .
	manualset3
144228	2	409171	5	NULL	NULL	0	NULL	HO-8910 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A showed the strongest inhibitory effect on HO-8910 ( IC50 = 21 microg/ml ) and Bel-7402 cells ( 16 mcirog/ml ) , whereas Fr .
	manualset3
144229	3	409171	5	NULL	NULL	0	NULL	IC50 = 21 microg/ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A showed the strongest inhibitory effect on HO-8910 ( IC50 = 21 microg/ml ) and Bel-7402 cells ( 16 mcirog/ml ) , whereas Fr .
	manualset3
144230	4	409171	5	NULL	NULL	0	NULL	Bel-7402 cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A showed the strongest inhibitory effect on HO-8910 ( IC50 = 21 microg/ml ) and Bel-7402 cells ( 16 mcirog/ml ) , whereas Fr .
	manualset3
144231	5	409171	5	NULL	NULL	0	NULL	16 mcirog/ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A showed the strongest inhibitory effect on HO-8910 ( IC50 = 21 microg/ml ) and Bel-7402 cells ( 16 mcirog/ml ) , whereas Fr .
	manualset3
144232	1	409172	5	NULL	NULL	0	NULL	clusters 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The clusters are located in the promoters and enhancers of genes , in introns , and in untranslated regions of the mRNA .
	manualset3
144233	2	409172	5	NULL	NULL	0	NULL	promoters 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The clusters are located in the promoters and enhancers of genes , in introns , and in untranslated regions of the mRNA .
	manualset3
144234	3	409172	5	NULL	NULL	0	NULL	enhancers 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The clusters are located in the promoters and enhancers of genes , in introns , and in untranslated regions of the mRNA .
	manualset3
144235	4	409172	5	NULL	NULL	0	NULL	genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The clusters are located in the promoters and enhancers of genes , in introns , and in untranslated regions of the mRNA .
	manualset3
144236	5	409172	5	NULL	NULL	0	NULL	introns 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The clusters are located in the promoters and enhancers of genes , in introns , and in untranslated regions of the mRNA .
	manualset3
144237	6	409172	5	NULL	NULL	0	NULL	untranslated regions 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The clusters are located in the promoters and enhancers of genes , in introns , and in untranslated regions of the mRNA .
	manualset3
144238	7	409172	5	NULL	NULL	0	NULL	mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The clusters are located in the promoters and enhancers of genes , in introns , and in untranslated regions of the mRNA .
	manualset3
144239	1	409173	5	NULL	NULL	0	NULL	co-expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The co-expression of GnT-III and ManII led to a similar degree of non-fucosylation as that obtained for Glyco-1 , but the majority of the oligosaccharides linked to this antibody ( `` Glyco-2 '' ) are of the complex type .
	manualset3
144240	2	409173	5	NULL	NULL	0	NULL	GnT-III	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The co-expression of GnT-III and ManII led to a similar degree of non-fucosylation as that obtained for Glyco-1 , but the majority of the oligosaccharides linked to this antibody ( `` Glyco-2 '' ) are of the complex type .
	manualset3
144241	3	409173	5	NULL	NULL	0	NULL	ManII 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The co-expression of GnT-III and ManII led to a similar degree of non-fucosylation as that obtained for Glyco-1 , but the majority of the oligosaccharides linked to this antibody ( `` Glyco-2 '' ) are of the complex type .
	manualset3
144242	4	409173	5	NULL	NULL	0	NULL	degree 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The co-expression of GnT-III and ManII led to a similar degree of non-fucosylation as that obtained for Glyco-1 , but the majority of the oligosaccharides linked to this antibody ( `` Glyco-2 '' ) are of the complex type .
	manualset3
144243	5	409173	5	NULL	NULL	0	NULL	non-fucosylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The co-expression of GnT-III and ManII led to a similar degree of non-fucosylation as that obtained for Glyco-1 , but the majority of the oligosaccharides linked to this antibody ( `` Glyco-2 '' ) are of the complex type .
	manualset3
144244	6	409173	5	NULL	NULL	0	NULL	Glyco-1	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The co-expression of GnT-III and ManII led to a similar degree of non-fucosylation as that obtained for Glyco-1 , but the majority of the oligosaccharides linked to this antibody ( `` Glyco-2 '' ) are of the complex type .
	manualset3
144245	7	409173	5	NULL	NULL	0	NULL	majority 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The co-expression of GnT-III and ManII led to a similar degree of non-fucosylation as that obtained for Glyco-1 , but the majority of the oligosaccharides linked to this antibody ( `` Glyco-2 '' ) are of the complex type .
	manualset3
144246	8	409173	5	NULL	NULL	0	NULL	oligosaccharides 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The co-expression of GnT-III and ManII led to a similar degree of non-fucosylation as that obtained for Glyco-1 , but the majority of the oligosaccharides linked to this antibody ( `` Glyco-2 '' ) are of the complex type .
	manualset3
144247	9	409173	5	NULL	NULL	0	NULL	antibody ( `` Glyco-2 '' ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The co-expression of GnT-III and ManII led to a similar degree of non-fucosylation as that obtained for Glyco-1 , but the majority of the oligosaccharides linked to this antibody ( `` Glyco-2 '' ) are of the complex type .
	manualset3
144248	10	409173	5	NULL	NULL	0	NULL	complex type	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The co-expression of GnT-III and ManII led to a similar degree of non-fucosylation as that obtained for Glyco-1 , but the majority of the oligosaccharides linked to this antibody ( `` Glyco-2 '' ) are of the complex type .
	manualset3
144249	1	409174	5	NULL	NULL	0	NULL	co-localization 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The co-localization and genetic interaction of Jag1 and Notch2 imply that this ligand and receptor physically interact , forming part of the signal transduction pathway required for glomerular differentiation and patterning .
	manualset3
144250	2	409174	5	NULL	NULL	0	NULL	genetic interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The co-localization and genetic interaction of Jag1 and Notch2 imply that this ligand and receptor physically interact , forming part of the signal transduction pathway required for glomerular differentiation and patterning .
	manualset3
144251	3	409174	5	NULL	NULL	0	NULL	Jag1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The co-localization and genetic interaction of Jag1 and Notch2 imply that this ligand and receptor physically interact , forming part of the signal transduction pathway required for glomerular differentiation and patterning .
	manualset3
144252	4	409174	5	NULL	NULL	0	NULL	Notch2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The co-localization and genetic interaction of Jag1 and Notch2 imply that this ligand and receptor physically interact , forming part of the signal transduction pathway required for glomerular differentiation and patterning .
	manualset3
144253	5	409174	5	NULL	NULL	0	NULL	Notch2 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The co-localization and genetic interaction of Jag1 and Notch2 imply that this ligand and receptor physically interact , forming part of the signal transduction pathway required for glomerular differentiation and patterning .
	manualset3
144254	6	409174	5	NULL	NULL	0	NULL	receptor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The co-localization and genetic interaction of Jag1 and Notch2 imply that this ligand and receptor physically interact , forming part of the signal transduction pathway required for glomerular differentiation and patterning .
	manualset3
144255	7	409174	5	NULL	NULL	0	NULL	signal transduction pathway 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The co-localization and genetic interaction of Jag1 and Notch2 imply that this ligand and receptor physically interact , forming part of the signal transduction pathway required for glomerular differentiation and patterning .
	manualset3
144256	8	409174	5	NULL	NULL	0	NULL	glomerular differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The co-localization and genetic interaction of Jag1 and Notch2 imply that this ligand and receptor physically interact , forming part of the signal transduction pathway required for glomerular differentiation and patterning .
	manualset3
144257	9	409174	5	NULL	NULL	0	NULL	patterning 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The co-localization and genetic interaction of Jag1 and Notch2 imply that this ligand and receptor physically interact , forming part of the signal transduction pathway required for glomerular differentiation and patterning .
	manualset3
144258	1	409175	5	NULL	NULL	0	NULL	coactivated left middle temporal gyrus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The coactivated left middle temporal gyrus further suggests that familiarity with a tool as well as the knowledge about its usage plays a role in peripersonal space modulation .
	manualset3
144259	2	409175	5	NULL	NULL	0	NULL	familiarity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The coactivated left middle temporal gyrus further suggests that familiarity with a tool as well as the knowledge about its usage plays a role in peripersonal space modulation .
	manualset3
144260	3	409175	5	NULL	NULL	0	NULL	tool 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The coactivated left middle temporal gyrus further suggests that familiarity with a tool as well as the knowledge about its usage plays a role in peripersonal space modulation .
	manualset3
144261	4	409175	5	NULL	NULL	NULL	NULL	knowledge 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The coactivated left middle temporal gyrus further suggests that familiarity with a tool as well as the knowledge about its usage plays a role in peripersonal space modulation .
	manualset3
144262	5	409175	5	NULL	NULL	0	NULL	usage 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The coactivated left middle temporal gyrus further suggests that familiarity with a tool as well as the knowledge about its usage plays a role in peripersonal space modulation .
	manualset3
144263	6	409175	5	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The coactivated left middle temporal gyrus further suggests that familiarity with a tool as well as the knowledge about its usage plays a role in peripersonal space modulation .
	manualset3
144264	7	409175	5	NULL	NULL	NULL	NULL	peripersonal space modulation	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The coactivated left middle temporal gyrus further suggests that familiarity with a tool as well as the knowledge about its usage plays a role in peripersonal space modulation .
	manualset3
144265	1	409176	5	NULL	NULL	0	NULL	coating 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The coating was performed on the inner surfaces of 50-200 microns sized pores and was also consistent in the smallest of the pores even those of 50 microns .
	manualset3
144266	2	409176	5	NULL	NULL	0	NULL	inner surfaces	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The coating was performed on the inner surfaces of 50-200 microns sized pores and was also consistent in the smallest of the pores even those of 50 microns .
	manualset3
144267	3	409176	5	NULL	NULL	0	NULL	 50-200 microns sized pores 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The coating was performed on the inner surfaces of 50-200 microns sized pores and was also consistent in the smallest of the pores even those of 50 microns .
	manualset3
144268	4	409176	5	NULL	NULL	0	NULL	pores 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The coating was performed on the inner surfaces of 50-200 microns sized pores and was also consistent in the smallest of the pores even those of 50 microns .
	manualset3
144269	5	409176	5	NULL	NULL	0	NULL	50 microns 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The coating was performed on the inner surfaces of 50-200 microns sized pores and was also consistent in the smallest of the pores even those of 50 microns .
	manualset3
144270	1	409177	5	NULL	NULL	0	NULL	coefficient of correlation 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The coefficient of correlation between urinary hGH in ng/h and post-clonidine peak was 0.50 ( P = 0.0015 ) , between urinary hGH in ng/l and post-clonidine peak was 0.48 ( P = 0.0025 ) , between urinary hGH in ng/l per hour and post-clonidine peak was 0.47 ( P = 0.0027 ) .
	manualset3
144271	2	409177	5	NULL	NULL	0	NULL	urinary hGH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The coefficient of correlation between urinary hGH in ng/h and post-clonidine peak was 0.50 ( P = 0.0015 ) , between urinary hGH in ng/l and post-clonidine peak was 0.48 ( P = 0.0025 ) , between urinary hGH in ng/l per hour and post-clonidine peak was 0.47 ( P = 0.0027 ) .
	manualset3
144272	3	409177	5	NULL	NULL	0	NULL	ng/h and post-clonidine peak	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The coefficient of correlation between urinary hGH in ng/h and post-clonidine peak was 0.50 ( P = 0.0015 ) , between urinary hGH in ng/l and post-clonidine peak was 0.48 ( P = 0.0025 ) , between urinary hGH in ng/l per hour and post-clonidine peak was 0.47 ( P = 0.0027 ) .
	manualset3
144273	4	409177	5	NULL	NULL	0	NULL	0.50 ( P = 0.0015 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The coefficient of correlation between urinary hGH in ng/h and post-clonidine peak was 0.50 ( P = 0.0015 ) , between urinary hGH in ng/l and post-clonidine peak was 0.48 ( P = 0.0025 ) , between urinary hGH in ng/l per hour and post-clonidine peak was 0.47 ( P = 0.0027 ) .
	manualset3
144274	5	409177	5	NULL	NULL	0	NULL	ng/l 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The coefficient of correlation between urinary hGH in ng/h and post-clonidine peak was 0.50 ( P = 0.0015 ) , between urinary hGH in ng/l and post-clonidine peak was 0.48 ( P = 0.0025 ) , between urinary hGH in ng/l per hour and post-clonidine peak was 0.47 ( P = 0.0027 ) .
	manualset3
144275	6	409177	5	NULL	NULL	0	NULL	post-clonidine peak	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The coefficient of correlation between urinary hGH in ng/h and post-clonidine peak was 0.50 ( P = 0.0015 ) , between urinary hGH in ng/l and post-clonidine peak was 0.48 ( P = 0.0025 ) , between urinary hGH in ng/l per hour and post-clonidine peak was 0.47 ( P = 0.0027 ) .
	manualset3
144276	7	409177	5	NULL	NULL	0	NULL	0.48 ( P = 0.0025 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The coefficient of correlation between urinary hGH in ng/h and post-clonidine peak was 0.50 ( P = 0.0015 ) , between urinary hGH in ng/l and post-clonidine peak was 0.48 ( P = 0.0025 ) , between urinary hGH in ng/l per hour and post-clonidine peak was 0.47 ( P = 0.0027 ) .
	manualset3
144277	8	409177	5	NULL	NULL	0	NULL	urinary hGH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The coefficient of correlation between urinary hGH in ng/h and post-clonidine peak was 0.50 ( P = 0.0015 ) , between urinary hGH in ng/l and post-clonidine peak was 0.48 ( P = 0.0025 ) , between urinary hGH in ng/l per hour and post-clonidine peak was 0.47 ( P = 0.0027 ) .
	manualset3
144278	9	409177	5	NULL	NULL	0	NULL	 ng/l per hour 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The coefficient of correlation between urinary hGH in ng/h and post-clonidine peak was 0.50 ( P = 0.0015 ) , between urinary hGH in ng/l and post-clonidine peak was 0.48 ( P = 0.0025 ) , between urinary hGH in ng/l per hour and post-clonidine peak was 0.47 ( P = 0.0027 ) .
	manualset3
144279	10	409177	5	NULL	NULL	0	NULL	post-clonidine peak	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The coefficient of correlation between urinary hGH in ng/h and post-clonidine peak was 0.50 ( P = 0.0015 ) , between urinary hGH in ng/l and post-clonidine peak was 0.48 ( P = 0.0025 ) , between urinary hGH in ng/l per hour and post-clonidine peak was 0.47 ( P = 0.0027 ) .
	manualset3
144280	11	409177	5	NULL	NULL	0	NULL	0.47 ( P = 0.0027 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The coefficient of correlation between urinary hGH in ng/h and post-clonidine peak was 0.50 ( P = 0.0015 ) , between urinary hGH in ng/l and post-clonidine peak was 0.48 ( P = 0.0025 ) , between urinary hGH in ng/l per hour and post-clonidine peak was 0.47 ( P = 0.0027 ) .
	manualset3
144281	1	409178	5	NULL	NULL	0	NULL	coefficient of variation	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The coefficient of variation in the width of `` islands '' of tumor cell mass is rather small ( 0.2 reverse similar0 .6 ) , implying the regularity of the spatial pattern .
	manualset3
144282	2	409178	5	NULL	NULL	0	NULL	width of `` islands ''	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The coefficient of variation in the width of `` islands '' of tumor cell mass is rather small ( 0.2 reverse similar0 .6 ) , implying the regularity of the spatial pattern .
	manualset3
144283	3	409178	5	NULL	NULL	0	NULL	tumor cell mass	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The coefficient of variation in the width of `` islands '' of tumor cell mass is rather small ( 0.2 reverse similar0 .6 ) , implying the regularity of the spatial pattern .
	manualset3
144284	4	409178	5	NULL	NULL	0	NULL	0.2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The coefficient of variation in the width of `` islands '' of tumor cell mass is rather small ( 0.2 reverse similar0 .6 ) , implying the regularity of the spatial pattern .
	manualset3
144285	5	409178	5	NULL	NULL	0	NULL	0 .6	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The coefficient of variation in the width of `` islands '' of tumor cell mass is rather small ( 0.2 reverse similar0 .6 ) , implying the regularity of the spatial pattern .
	manualset3
144286	6	409178	5	NULL	NULL	0	NULL	regularity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The coefficient of variation in the width of `` islands '' of tumor cell mass is rather small ( 0.2 reverse similar0 .6 ) , implying the regularity of the spatial pattern .
	manualset3
144287	7	409178	5	NULL	NULL	0	NULL	spatial pattern 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The coefficient of variation in the width of `` islands '' of tumor cell mass is rather small ( 0.2 reverse similar0 .6 ) , implying the regularity of the spatial pattern .
	manualset3
144288	1	409179	5	NULL	NULL	0	NULL	coexistence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The coexistence of pemphigus and bullous pemphigoid is very uncommon .
	manualset3
144289	2	409179	5	NULL	NULL	0	NULL	pemphigus 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The coexistence of pemphigus and bullous pemphigoid is very uncommon .
	manualset3
144290	3	409179	5	NULL	NULL	0	NULL	bullous pemphigoid 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The coexistence of pemphigus and bullous pemphigoid is very uncommon .
	manualset3
144291	1	409180	5	NULL	NULL	0	NULL	cognitive function	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cognitive function of memory , but not that of attention , was impaired , also starting at the 4.4-mM glucose step .
	manualset3
144292	2	409180	5	NULL	NULL	0	NULL	memory 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cognitive function of memory , but not that of attention , was impaired , also starting at the 4.4-mM glucose step .
	manualset3
144293	3	409180	5	NULL	NULL	0	NULL	attention 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cognitive function of memory , but not that of attention , was impaired , also starting at the 4.4-mM glucose step .
	manualset3
144294	4	409180	5	NULL	NULL	0	NULL	4.4-mM glucose step	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cognitive function of memory , but not that of attention , was impaired , also starting at the 4.4-mM glucose step .
	manualset3
144295	1	409181	5	NULL	NULL	0	NULL	collagen membrane	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The collagen membrane forms the roof of a ` biological chamber ' , and serves to protect and contains the stem cells as they differentiate into chondrocytes , which will form a healthy regenerative cartilage .
	manualset3
144296	2	409181	5	NULL	NULL	0	NULL	biological chamber	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The collagen membrane forms the roof of a ` biological chamber ' , and serves to protect and contains the stem cells as they differentiate into chondrocytes , which will form a healthy regenerative cartilage .
	manualset3
144297	3	409181	5	NULL	NULL	0	NULL	stem cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The collagen membrane forms the roof of a ` biological chamber ' , and serves to protect and contains the stem cells as they differentiate into chondrocytes , which will form a healthy regenerative cartilage .
	manualset3
144298	4	409181	5	NULL	NULL	0	NULL	chondrocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The collagen membrane forms the roof of a ` biological chamber ' , and serves to protect and contains the stem cells as they differentiate into chondrocytes , which will form a healthy regenerative cartilage .
	manualset3
144299	5	409181	5	NULL	NULL	0	NULL	healthy regenerative cartilage	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The collagen membrane forms the roof of a ` biological chamber ' , and serves to protect and contains the stem cells as they differentiate into chondrocytes , which will form a healthy regenerative cartilage .
	manualset3
144300	1	409182	5	NULL	NULL	0	NULL	collection 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The collection rapidly decreased after worm treatment .
	manualset3
144301	2	409182	5	NULL	NULL	0	NULL	worm treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The collection rapidly decreased after worm treatment .
	manualset3
144302	1	409183	5	NULL	NULL	0	NULL	colony morphology/size	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The colony morphology/size , AA , and HP characteristics are expressed in both Y. pseudotuberculosis and Y. enterocolitica but not in Y. pestis .
	manualset3
144303	2	409183	5	NULL	NULL	0	NULL	AA 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The colony morphology/size , AA , and HP characteristics are expressed in both Y. pseudotuberculosis and Y. enterocolitica but not in Y. pestis .
	manualset3
144304	3	409183	5	NULL	NULL	0	NULL	HP characteristics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The colony morphology/size , AA , and HP characteristics are expressed in both Y. pseudotuberculosis and Y. enterocolitica but not in Y. pestis .
	manualset3
144305	4	409183	5	NULL	NULL	0	NULL	Y. pseudotuberculosis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The colony morphology/size , AA , and HP characteristics are expressed in both Y. pseudotuberculosis and Y. enterocolitica but not in Y. pestis .
	manualset3
144306	5	409183	5	NULL	NULL	0	NULL	Y. enterocolitica 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The colony morphology/size , AA , and HP characteristics are expressed in both Y. pseudotuberculosis and Y. enterocolitica but not in Y. pestis .
	manualset3
144307	6	409183	5	NULL	NULL	0	NULL	Y. pestis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The colony morphology/size , AA , and HP characteristics are expressed in both Y. pseudotuberculosis and Y. enterocolitica but not in Y. pestis .
	manualset3
144308	1	409184	5	NULL	NULL	0	NULL	color coding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The color coding offers the possibility to identify any radiographic changes that take place over time , eg , growth , apposition or resorption of bone , and progression or regression of pathological processes .
	manualset3
144309	2	409184	5	NULL	NULL	0	NULL	possibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The color coding offers the possibility to identify any radiographic changes that take place over time , eg , growth , apposition or resorption of bone , and progression or regression of pathological processes .
	manualset3
144310	3	409184	5	NULL	NULL	0	NULL	radiographic changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The color coding offers the possibility to identify any radiographic changes that take place over time , eg , growth , apposition or resorption of bone , and progression or regression of pathological processes .
	manualset3
144311	4	409184	5	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The color coding offers the possibility to identify any radiographic changes that take place over time , eg , growth , apposition or resorption of bone , and progression or regression of pathological processes .
	manualset3
144312	5	409184	5	NULL	NULL	0	NULL	growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The color coding offers the possibility to identify any radiographic changes that take place over time , eg , growth , apposition or resorption of bone , and progression or regression of pathological processes .
	manualset3
144313	6	409184	5	NULL	NULL	0	NULL	apposition 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The color coding offers the possibility to identify any radiographic changes that take place over time , eg , growth , apposition or resorption of bone , and progression or regression of pathological processes .
	manualset3
144314	7	409184	5	NULL	NULL	0	NULL	resorption 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The color coding offers the possibility to identify any radiographic changes that take place over time , eg , growth , apposition or resorption of bone , and progression or regression of pathological processes .
	manualset3
144315	8	409184	5	NULL	NULL	0	NULL	bone 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The color coding offers the possibility to identify any radiographic changes that take place over time , eg , growth , apposition or resorption of bone , and progression or regression of pathological processes .
	manualset3
144316	9	409184	5	NULL	NULL	0	NULL	progression 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The color coding offers the possibility to identify any radiographic changes that take place over time , eg , growth , apposition or resorption of bone , and progression or regression of pathological processes .
	manualset3
144317	10	409184	5	NULL	NULL	0	NULL	regression 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The color coding offers the possibility to identify any radiographic changes that take place over time , eg , growth , apposition or resorption of bone , and progression or regression of pathological processes .
	manualset3
144318	11	409184	5	NULL	NULL	0	NULL	pathological processes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The color coding offers the possibility to identify any radiographic changes that take place over time , eg , growth , apposition or resorption of bone , and progression or regression of pathological processes .
	manualset3
144319	1	409185	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of 5 % NAC and 5 % TX-100 significantly enhanced the nasal , the pulmonary and the large intestinal absorption of FD-4 compared to the control , and the enhancement ratios relative to the control were 7.2 - , 2.8 - and 4.5-fold , respectively .
	manualset3
144320	2	409185	5	NULL	NULL	0	NULL	 5 % NAC	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of 5 % NAC and 5 % TX-100 significantly enhanced the nasal , the pulmonary and the large intestinal absorption of FD-4 compared to the control , and the enhancement ratios relative to the control were 7.2 - , 2.8 - and 4.5-fold , respectively .
	manualset3
144321	3	409185	5	NULL	NULL	0	NULL	5 % TX-100 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of 5 % NAC and 5 % TX-100 significantly enhanced the nasal , the pulmonary and the large intestinal absorption of FD-4 compared to the control , and the enhancement ratios relative to the control were 7.2 - , 2.8 - and 4.5-fold , respectively .
	manualset3
144322	4	409185	5	NULL	NULL	0	NULL	nasal absorption 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of 5 % NAC and 5 % TX-100 significantly enhanced the nasal , the pulmonary and the large intestinal absorption of FD-4 compared to the control , and the enhancement ratios relative to the control were 7.2 - , 2.8 - and 4.5-fold , respectively .
	manualset3
144323	5	409185	5	NULL	NULL	0	NULL	pulmonary absorption 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of 5 % NAC and 5 % TX-100 significantly enhanced the nasal , the pulmonary and the large intestinal absorption of FD-4 compared to the control , and the enhancement ratios relative to the control were 7.2 - , 2.8 - and 4.5-fold , respectively .
	manualset3
144324	6	409185	5	NULL	NULL	0	NULL	FD-4	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of 5 % NAC and 5 % TX-100 significantly enhanced the nasal , the pulmonary and the large intestinal absorption of FD-4 compared to the control , and the enhancement ratios relative to the control were 7.2 - , 2.8 - and 4.5-fold , respectively .
	manualset3
144325	7	409185	5	NULL	NULL	0	NULL	control 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of 5 % NAC and 5 % TX-100 significantly enhanced the nasal , the pulmonary and the large intestinal absorption of FD-4 compared to the control , and the enhancement ratios relative to the control were 7.2 - , 2.8 - and 4.5-fold , respectively .
	manualset3
144326	8	409185	5	NULL	NULL	0	NULL	enhancement ratios 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of 5 % NAC and 5 % TX-100 significantly enhanced the nasal , the pulmonary and the large intestinal absorption of FD-4 compared to the control , and the enhancement ratios relative to the control were 7.2 - , 2.8 - and 4.5-fold , respectively .
	manualset3
144327	9	409185	5	NULL	NULL	0	NULL	control 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of 5 % NAC and 5 % TX-100 significantly enhanced the nasal , the pulmonary and the large intestinal absorption of FD-4 compared to the control , and the enhancement ratios relative to the control were 7.2 - , 2.8 - and 4.5-fold , respectively .
	manualset3
144328	10	409185	5	NULL	NULL	0	NULL	7.2 - fold	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of 5 % NAC and 5 % TX-100 significantly enhanced the nasal , the pulmonary and the large intestinal absorption of FD-4 compared to the control , and the enhancement ratios relative to the control were 7.2 - , 2.8 - and 4.5-fold , respectively .
	manualset3
144329	11	409185	5	NULL	NULL	0	NULL	2.8 - fold 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of 5 % NAC and 5 % TX-100 significantly enhanced the nasal , the pulmonary and the large intestinal absorption of FD-4 compared to the control , and the enhancement ratios relative to the control were 7.2 - , 2.8 - and 4.5-fold , respectively .
	manualset3
144330	12	409185	5	NULL	NULL	0	NULL	4.5-fold 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of 5 % NAC and 5 % TX-100 significantly enhanced the nasal , the pulmonary and the large intestinal absorption of FD-4 compared to the control , and the enhancement ratios relative to the control were 7.2 - , 2.8 - and 4.5-fold , respectively .
	manualset3
144331	1	409186	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of DUP 753 and cyclosporin CSA abolished the CSA-induced increase in angiotensin receptor density in all four organs .
	manualset3
144332	2	409186	5	NULL	NULL	0	NULL	DUP 753 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of DUP 753 and cyclosporin CSA abolished the CSA-induced increase in angiotensin receptor density in all four organs .
	manualset3
144333	3	409186	5	NULL	NULL	0	NULL	cyclosporin CSA	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of DUP 753 and cyclosporin CSA abolished the CSA-induced increase in angiotensin receptor density in all four organs .
	manualset3
144334	4	409186	5	NULL	NULL	0	NULL	CSA-induced increase in angiotensin receptor density	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of DUP 753 and cyclosporin CSA abolished the CSA-induced increase in angiotensin receptor density in all four organs .
	manualset3
144335	5	409186	5	NULL	NULL	0	NULL	four 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of DUP 753 and cyclosporin CSA abolished the CSA-induced increase in angiotensin receptor density in all four organs .
	manualset3
144336	6	409186	5	NULL	NULL	0	NULL	organs 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of DUP 753 and cyclosporin CSA abolished the CSA-induced increase in angiotensin receptor density in all four organs .
	manualset3
144337	1	409187	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of E2 and E7 has the advantage that E2 is expressed in early dysplasia and neoplasia lesions , where E7 is expressed in more advance lesions .
	manualset3
144338	2	409187	5	NULL	NULL	0	NULL	E2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of E2 and E7 has the advantage that E2 is expressed in early dysplasia and neoplasia lesions , where E7 is expressed in more advance lesions .
	manualset3
144339	3	409187	5	NULL	NULL	0	NULL	E7 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of E2 and E7 has the advantage that E2 is expressed in early dysplasia and neoplasia lesions , where E7 is expressed in more advance lesions .
	manualset3
144340	4	409187	5	NULL	NULL	0	NULL	E2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of E2 and E7 has the advantage that E2 is expressed in early dysplasia and neoplasia lesions , where E7 is expressed in more advance lesions .
	manualset3
144341	5	409187	5	NULL	NULL	0	NULL	early dysplasia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of E2 and E7 has the advantage that E2 is expressed in early dysplasia and neoplasia lesions , where E7 is expressed in more advance lesions .
	manualset3
144342	6	409187	5	NULL	NULL	0	NULL	neoplasia lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of E2 and E7 has the advantage that E2 is expressed in early dysplasia and neoplasia lesions , where E7 is expressed in more advance lesions .
	manualset3
144343	7	409187	5	NULL	NULL	0	NULL	E7 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of E2 and E7 has the advantage that E2 is expressed in early dysplasia and neoplasia lesions , where E7 is expressed in more advance lesions .
	manualset3
144344	8	409187	5	NULL	NULL	0	NULL	advance lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of E2 and E7 has the advantage that E2 is expressed in early dysplasia and neoplasia lesions , where E7 is expressed in more advance lesions .
	manualset3
144345	1	409188	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of LAMB ( 40 mg/kg/day ) and G-CSF ( 150 or 300 microg/kg/day ) did not improve the results obtained with LAMB alone .
	manualset3
144346	2	409188	5	NULL	NULL	0	NULL	LAMB 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of LAMB ( 40 mg/kg/day ) and G-CSF ( 150 or 300 microg/kg/day ) did not improve the results obtained with LAMB alone .
	manualset3
144347	3	409188	5	NULL	NULL	0	NULL	40 mg/kg/day 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of LAMB ( 40 mg/kg/day ) and G-CSF ( 150 or 300 microg/kg/day ) did not improve the results obtained with LAMB alone .
	manualset3
144348	4	409188	5	NULL	NULL	NULL	NULL	G-CSF 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The combination of LAMB ( 40 mg/kg/day ) and G-CSF ( 150 or 300 microg/kg/day ) did not improve the results obtained with LAMB alone .
	manualset3
144349	5	409188	5	NULL	NULL	0	NULL	 150 or 300 microg/kg/day 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of LAMB ( 40 mg/kg/day ) and G-CSF ( 150 or 300 microg/kg/day ) did not improve the results obtained with LAMB alone .
	manualset3
144350	6	409188	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of LAMB ( 40 mg/kg/day ) and G-CSF ( 150 or 300 microg/kg/day ) did not improve the results obtained with LAMB alone .
	manualset3
144351	7	409188	5	NULL	NULL	0	NULL	LAMB 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of LAMB ( 40 mg/kg/day ) and G-CSF ( 150 or 300 microg/kg/day ) did not improve the results obtained with LAMB alone .
	manualset3
144352	1	409189	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of PA and soybean oil supplementation yielded essentially the same results as the diet containing the good corn .
	manualset3
144353	2	409189	5	NULL	NULL	0	NULL	PA 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of PA and soybean oil supplementation yielded essentially the same results as the diet containing the good corn .
	manualset3
144354	3	409189	5	NULL	NULL	0	NULL	soybean oil supplementation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of PA and soybean oil supplementation yielded essentially the same results as the diet containing the good corn .
	manualset3
144355	4	409189	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of PA and soybean oil supplementation yielded essentially the same results as the diet containing the good corn .
	manualset3
144356	5	409189	5	NULL	NULL	0	NULL	diet 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of PA and soybean oil supplementation yielded essentially the same results as the diet containing the good corn .
	manualset3
144357	6	409189	5	NULL	NULL	0	NULL	good corn	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of PA and soybean oil supplementation yielded essentially the same results as the diet containing the good corn .
	manualset3
144358	1	409190	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of level of urinary 8-oxodG below the median and hepatitis B virus infection resulted in an OR of 11.4 ( 95 % CI 3.9-33 .3 ) , compared with those with urinary 8-oxodG above the median and hepatitis B virus surface antigen negative .
	manualset3
144359	2	409190	5	NULL	NULL	0	NULL	level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of level of urinary 8-oxodG below the median and hepatitis B virus infection resulted in an OR of 11.4 ( 95 % CI 3.9-33 .3 ) , compared with those with urinary 8-oxodG above the median and hepatitis B virus surface antigen negative .
	manualset3
144360	3	409190	5	NULL	NULL	0	NULL	urinary 8-oxodG 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of level of urinary 8-oxodG below the median and hepatitis B virus infection resulted in an OR of 11.4 ( 95 % CI 3.9-33 .3 ) , compared with those with urinary 8-oxodG above the median and hepatitis B virus surface antigen negative .
	manualset3
144361	4	409190	5	NULL	NULL	0	NULL	hepatitis B virus infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of level of urinary 8-oxodG below the median and hepatitis B virus infection resulted in an OR of 11.4 ( 95 % CI 3.9-33 .3 ) , compared with those with urinary 8-oxodG above the median and hepatitis B virus surface antigen negative .
	manualset3
144362	5	409190	5	NULL	NULL	0	NULL	OR 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of level of urinary 8-oxodG below the median and hepatitis B virus infection resulted in an OR of 11.4 ( 95 % CI 3.9-33 .3 ) , compared with those with urinary 8-oxodG above the median and hepatitis B virus surface antigen negative .
	manualset3
144363	6	409190	5	NULL	NULL	0	NULL	11.4 ( 95 % CI 3.9-33 .3 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of level of urinary 8-oxodG below the median and hepatitis B virus infection resulted in an OR of 11.4 ( 95 % CI 3.9-33 .3 ) , compared with those with urinary 8-oxodG above the median and hepatitis B virus surface antigen negative .
	manualset3
144364	7	409190	5	NULL	NULL	0	NULL	urinary 8-oxodG	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of level of urinary 8-oxodG below the median and hepatitis B virus infection resulted in an OR of 11.4 ( 95 % CI 3.9-33 .3 ) , compared with those with urinary 8-oxodG above the median and hepatitis B virus surface antigen negative .
	manualset3
144365	8	409190	5	NULL	NULL	0	NULL	hepatitis B virus surface antigen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of level of urinary 8-oxodG below the median and hepatitis B virus infection resulted in an OR of 11.4 ( 95 % CI 3.9-33 .3 ) , compared with those with urinary 8-oxodG above the median and hepatitis B virus surface antigen negative .
	manualset3
144366	1	409191	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of marble sludge and compost was most effective at diminishing toxicity in lettuce .
	manualset3
144367	2	409191	5	NULL	NULL	0	NULL	 marble sludge 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of marble sludge and compost was most effective at diminishing toxicity in lettuce .
	manualset3
144368	3	409191	5	NULL	NULL	0	NULL	compost 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of marble sludge and compost was most effective at diminishing toxicity in lettuce .
	manualset3
144369	4	409191	5	NULL	NULL	0	NULL	toxicity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of marble sludge and compost was most effective at diminishing toxicity in lettuce .
	manualset3
144370	5	409191	5	NULL	NULL	0	NULL	lettuce 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of marble sludge and compost was most effective at diminishing toxicity in lettuce .
	manualset3
144371	1	409192	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the Glu-A1b , Glu-B1c , and Glu-D1a alleles prevails among the spring cultivars , and the combination of the Glu-A1a , Glu-B1c , and Glu-D1d alleles prevails among the winter cultivars .
	manualset3
144372	2	409192	5	NULL	NULL	0	NULL	Glu-A1b alleles 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the Glu-A1b , Glu-B1c , and Glu-D1a alleles prevails among the spring cultivars , and the combination of the Glu-A1a , Glu-B1c , and Glu-D1d alleles prevails among the winter cultivars .
	manualset3
144373	3	409192	5	NULL	NULL	0	NULL	Glu-B1c alleles 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the Glu-A1b , Glu-B1c , and Glu-D1a alleles prevails among the spring cultivars , and the combination of the Glu-A1a , Glu-B1c , and Glu-D1d alleles prevails among the winter cultivars .
	manualset3
144374	4	409192	5	NULL	NULL	0	NULL	 Glu-D1a alleles 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the Glu-A1b , Glu-B1c , and Glu-D1a alleles prevails among the spring cultivars , and the combination of the Glu-A1a , Glu-B1c , and Glu-D1d alleles prevails among the winter cultivars .
	manualset3
144375	5	409192	5	NULL	NULL	0	NULL	spring cultivars	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the Glu-A1b , Glu-B1c , and Glu-D1a alleles prevails among the spring cultivars , and the combination of the Glu-A1a , Glu-B1c , and Glu-D1d alleles prevails among the winter cultivars .
	manualset3
144376	6	409192	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the Glu-A1b , Glu-B1c , and Glu-D1a alleles prevails among the spring cultivars , and the combination of the Glu-A1a , Glu-B1c , and Glu-D1d alleles prevails among the winter cultivars .
	manualset3
144377	7	409192	5	NULL	NULL	0	NULL	Glu-A1a alleles 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the Glu-A1b , Glu-B1c , and Glu-D1a alleles prevails among the spring cultivars , and the combination of the Glu-A1a , Glu-B1c , and Glu-D1d alleles prevails among the winter cultivars .
	manualset3
144378	8	409192	5	NULL	NULL	0	NULL	Glu-B1c alleles 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the Glu-A1b , Glu-B1c , and Glu-D1a alleles prevails among the spring cultivars , and the combination of the Glu-A1a , Glu-B1c , and Glu-D1d alleles prevails among the winter cultivars .
	manualset3
144379	9	409192	5	NULL	NULL	0	NULL	Glu-D1d alleles 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the Glu-A1b , Glu-B1c , and Glu-D1a alleles prevails among the spring cultivars , and the combination of the Glu-A1a , Glu-B1c , and Glu-D1d alleles prevails among the winter cultivars .
	manualset3
144380	10	409192	5	NULL	NULL	0	NULL	winter cultivars	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the Glu-A1b , Glu-B1c , and Glu-D1a alleles prevails among the spring cultivars , and the combination of the Glu-A1a , Glu-B1c , and Glu-D1d alleles prevails among the winter cultivars .
	manualset3
144381	1	409193	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the Neurosurgical Log-book and the new Evaluation Sheet allows a comprehensive assessment of the knowledge , progress , as well as the personal and professional development of the individual resident .
	manualset3
144382	2	409193	5	NULL	NULL	0	NULL	Neurosurgical Log-book 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the Neurosurgical Log-book and the new Evaluation Sheet allows a comprehensive assessment of the knowledge , progress , as well as the personal and professional development of the individual resident .
	manualset3
144383	3	409193	5	NULL	NULL	0	NULL	Evaluation Sheet 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the Neurosurgical Log-book and the new Evaluation Sheet allows a comprehensive assessment of the knowledge , progress , as well as the personal and professional development of the individual resident .
	manualset3
144384	4	409193	5	NULL	NULL	0	NULL	comprehensive assessment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the Neurosurgical Log-book and the new Evaluation Sheet allows a comprehensive assessment of the knowledge , progress , as well as the personal and professional development of the individual resident .
	manualset3
144385	5	409193	5	NULL	NULL	0	NULL	knowledge 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the Neurosurgical Log-book and the new Evaluation Sheet allows a comprehensive assessment of the knowledge , progress , as well as the personal and professional development of the individual resident .
	manualset3
144386	6	409193	5	NULL	NULL	0	NULL	progress 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the Neurosurgical Log-book and the new Evaluation Sheet allows a comprehensive assessment of the knowledge , progress , as well as the personal and professional development of the individual resident .
	manualset3
144387	7	409193	5	NULL	NULL	0	NULL	personal development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the Neurosurgical Log-book and the new Evaluation Sheet allows a comprehensive assessment of the knowledge , progress , as well as the personal and professional development of the individual resident .
	manualset3
144388	8	409193	5	NULL	NULL	0	NULL	 professional development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the Neurosurgical Log-book and the new Evaluation Sheet allows a comprehensive assessment of the knowledge , progress , as well as the personal and professional development of the individual resident .
	manualset3
144389	9	409193	5	NULL	NULL	0	NULL	individual resident	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the Neurosurgical Log-book and the new Evaluation Sheet allows a comprehensive assessment of the knowledge , progress , as well as the personal and professional development of the individual resident .
	manualset3
144390	1	409194	5	NULL	NULL	NULL	NULL	significant clinical alteration	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A significant clinical alteration of the VOR during VNS was not observed .
	manualset3
144391	2	409194	5	NULL	NULL	0	NULL	VOR 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant clinical alteration of the VOR during VNS was not observed .
	manualset3
144392	3	409194	5	NULL	NULL	NULL	NULL	VNS 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A significant clinical alteration of the VOR during VNS was not observed .
	manualset3
144393	1	409195	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the TSA and sABC amplification systems provided the first successful co-localization of sympathetic adrenergic and sympathetic cholinergic nerve fibers in cutaneous human sweat glands and vasomotor and pilomotor systems .
	manualset3
144394	2	409195	5	NULL	NULL	0	NULL	TSA amplification systems	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the TSA and sABC amplification systems provided the first successful co-localization of sympathetic adrenergic and sympathetic cholinergic nerve fibers in cutaneous human sweat glands and vasomotor and pilomotor systems .
	manualset3
144395	3	409195	5	NULL	NULL	0	NULL	sABC amplification systems	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the TSA and sABC amplification systems provided the first successful co-localization of sympathetic adrenergic and sympathetic cholinergic nerve fibers in cutaneous human sweat glands and vasomotor and pilomotor systems .
	manualset3
144396	4	409195	5	NULL	NULL	0	NULL	 co-localization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the TSA and sABC amplification systems provided the first successful co-localization of sympathetic adrenergic and sympathetic cholinergic nerve fibers in cutaneous human sweat glands and vasomotor and pilomotor systems .
	manualset3
144397	5	409195	5	NULL	NULL	0	NULL	adrenergic nerve fibers	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the TSA and sABC amplification systems provided the first successful co-localization of sympathetic adrenergic and sympathetic cholinergic nerve fibers in cutaneous human sweat glands and vasomotor and pilomotor systems .
	manualset3
144398	6	409195	5	NULL	NULL	0	NULL	sympathetic cholinergic nerve fibers	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the TSA and sABC amplification systems provided the first successful co-localization of sympathetic adrenergic and sympathetic cholinergic nerve fibers in cutaneous human sweat glands and vasomotor and pilomotor systems .
	manualset3
144399	7	409195	5	NULL	NULL	0	NULL	cutaneous human sweat glands	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the TSA and sABC amplification systems provided the first successful co-localization of sympathetic adrenergic and sympathetic cholinergic nerve fibers in cutaneous human sweat glands and vasomotor and pilomotor systems .
	manualset3
144400	8	409195	5	NULL	NULL	0	NULL	vasomotor system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the TSA and sABC amplification systems provided the first successful co-localization of sympathetic adrenergic and sympathetic cholinergic nerve fibers in cutaneous human sweat glands and vasomotor and pilomotor systems .
	manualset3
144401	9	409195	5	NULL	NULL	0	NULL	pilomotor system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the TSA and sABC amplification systems provided the first successful co-localization of sympathetic adrenergic and sympathetic cholinergic nerve fibers in cutaneous human sweat glands and vasomotor and pilomotor systems .
	manualset3
144402	1	409196	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the above pathogens in the rectum were the following : gonococci and chlamydia ( 15 per cent of the cases ) , gonococci , chlamydia and Trichomonas ( 7.3 per cent ) , gonococci and ureaplasma ( 7.3 per cent ) , ureaplasma and chlamydia ( 7.8 per cent ) .
	manualset3
144403	2	409196	5	NULL	NULL	0	NULL	pathogens 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the above pathogens in the rectum were the following : gonococci and chlamydia ( 15 per cent of the cases ) , gonococci , chlamydia and Trichomonas ( 7.3 per cent ) , gonococci and ureaplasma ( 7.3 per cent ) , ureaplasma and chlamydia ( 7.8 per cent ) .
	manualset3
144404	3	409196	5	NULL	NULL	0	NULL	rectum 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the above pathogens in the rectum were the following : gonococci and chlamydia ( 15 per cent of the cases ) , gonococci , chlamydia and Trichomonas ( 7.3 per cent ) , gonococci and ureaplasma ( 7.3 per cent ) , ureaplasma and chlamydia ( 7.8 per cent ) .
	manualset3
144405	4	409196	5	NULL	NULL	0	NULL	gonococci 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the above pathogens in the rectum were the following : gonococci and chlamydia ( 15 per cent of the cases ) , gonococci , chlamydia and Trichomonas ( 7.3 per cent ) , gonococci and ureaplasma ( 7.3 per cent ) , ureaplasma and chlamydia ( 7.8 per cent ) .
	manualset3
144406	5	409196	5	NULL	NULL	0	NULL	chlamydia 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the above pathogens in the rectum were the following : gonococci and chlamydia ( 15 per cent of the cases ) , gonococci , chlamydia and Trichomonas ( 7.3 per cent ) , gonococci and ureaplasma ( 7.3 per cent ) , ureaplasma and chlamydia ( 7.8 per cent ) .
	manualset3
144407	6	409196	5	NULL	NULL	0	NULL	15 per cent of the cases	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the above pathogens in the rectum were the following : gonococci and chlamydia ( 15 per cent of the cases ) , gonococci , chlamydia and Trichomonas ( 7.3 per cent ) , gonococci and ureaplasma ( 7.3 per cent ) , ureaplasma and chlamydia ( 7.8 per cent ) .
	manualset3
144408	7	409196	5	NULL	NULL	0	NULL	gonococci 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the above pathogens in the rectum were the following : gonococci and chlamydia ( 15 per cent of the cases ) , gonococci , chlamydia and Trichomonas ( 7.3 per cent ) , gonococci and ureaplasma ( 7.3 per cent ) , ureaplasma and chlamydia ( 7.8 per cent ) .
	manualset3
144409	8	409196	5	NULL	NULL	0	NULL	chlamydia 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the above pathogens in the rectum were the following : gonococci and chlamydia ( 15 per cent of the cases ) , gonococci , chlamydia and Trichomonas ( 7.3 per cent ) , gonococci and ureaplasma ( 7.3 per cent ) , ureaplasma and chlamydia ( 7.8 per cent ) .
	manualset3
144410	9	409196	5	NULL	NULL	0	NULL	Trichomonas 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the above pathogens in the rectum were the following : gonococci and chlamydia ( 15 per cent of the cases ) , gonococci , chlamydia and Trichomonas ( 7.3 per cent ) , gonococci and ureaplasma ( 7.3 per cent ) , ureaplasma and chlamydia ( 7.8 per cent ) .
	manualset3
144411	10	409196	5	NULL	NULL	0	NULL	 7.3 per cent	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the above pathogens in the rectum were the following : gonococci and chlamydia ( 15 per cent of the cases ) , gonococci , chlamydia and Trichomonas ( 7.3 per cent ) , gonococci and ureaplasma ( 7.3 per cent ) , ureaplasma and chlamydia ( 7.8 per cent ) .
	manualset3
144412	11	409196	5	NULL	NULL	0	NULL	gonococci 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the above pathogens in the rectum were the following : gonococci and chlamydia ( 15 per cent of the cases ) , gonococci , chlamydia and Trichomonas ( 7.3 per cent ) , gonococci and ureaplasma ( 7.3 per cent ) , ureaplasma and chlamydia ( 7.8 per cent ) .
	manualset3
144413	12	409196	5	NULL	NULL	0	NULL	ureaplasma 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the above pathogens in the rectum were the following : gonococci and chlamydia ( 15 per cent of the cases ) , gonococci , chlamydia and Trichomonas ( 7.3 per cent ) , gonococci and ureaplasma ( 7.3 per cent ) , ureaplasma and chlamydia ( 7.8 per cent ) .
	manualset3
144414	13	409196	5	NULL	NULL	0	NULL	7.3 per cent	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the above pathogens in the rectum were the following : gonococci and chlamydia ( 15 per cent of the cases ) , gonococci , chlamydia and Trichomonas ( 7.3 per cent ) , gonococci and ureaplasma ( 7.3 per cent ) , ureaplasma and chlamydia ( 7.8 per cent ) .
	manualset3
144415	14	409196	5	NULL	NULL	0	NULL	ureaplasma 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the above pathogens in the rectum were the following : gonococci and chlamydia ( 15 per cent of the cases ) , gonococci , chlamydia and Trichomonas ( 7.3 per cent ) , gonococci and ureaplasma ( 7.3 per cent ) , ureaplasma and chlamydia ( 7.8 per cent ) .
	manualset3
144416	15	409196	5	NULL	NULL	0	NULL	chlamydia 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the above pathogens in the rectum were the following : gonococci and chlamydia ( 15 per cent of the cases ) , gonococci , chlamydia and Trichomonas ( 7.3 per cent ) , gonococci and ureaplasma ( 7.3 per cent ) , ureaplasma and chlamydia ( 7.8 per cent ) .
	manualset3
144417	16	409196	5	NULL	NULL	0	NULL	7.8 per cent	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the above pathogens in the rectum were the following : gonococci and chlamydia ( 15 per cent of the cases ) , gonococci , chlamydia and Trichomonas ( 7.3 per cent ) , gonococci and ureaplasma ( 7.3 per cent ) , ureaplasma and chlamydia ( 7.8 per cent ) .
	manualset3
144418	1	409197	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the two parameters ( contraction index , CI ) provided a realistic evaluation of the contractile capacities of the cell population of the cultures as a whole .
	manualset3
144419	2	409197	5	NULL	NULL	0	NULL	two parameters	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the two parameters ( contraction index , CI ) provided a realistic evaluation of the contractile capacities of the cell population of the cultures as a whole .
	manualset3
144420	3	409197	5	NULL	NULL	0	NULL	contraction index , CI	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the two parameters ( contraction index , CI ) provided a realistic evaluation of the contractile capacities of the cell population of the cultures as a whole .
	manualset3
144421	4	409197	5	NULL	NULL	0	NULL	realistic evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the two parameters ( contraction index , CI ) provided a realistic evaluation of the contractile capacities of the cell population of the cultures as a whole .
	manualset3
144422	5	409197	5	NULL	NULL	0	NULL	contractile capacities 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the two parameters ( contraction index , CI ) provided a realistic evaluation of the contractile capacities of the cell population of the cultures as a whole .
	manualset3
144423	6	409197	5	NULL	NULL	0	NULL	cell population	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the two parameters ( contraction index , CI ) provided a realistic evaluation of the contractile capacities of the cell population of the cultures as a whole .
	manualset3
144424	7	409197	5	NULL	NULL	0	NULL	cultures 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of the two parameters ( contraction index , CI ) provided a realistic evaluation of the contractile capacities of the cell population of the cultures as a whole .
	manualset3
144425	1	409198	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of unstable angina with signs of coronary spasm is the least favorable ANO variant in terms of the risk of grave ventricular arrhythmias .
	manualset3
144426	2	409198	5	NULL	NULL	0	NULL	unstable angina 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of unstable angina with signs of coronary spasm is the least favorable ANO variant in terms of the risk of grave ventricular arrhythmias .
	manualset3
144427	3	409198	5	NULL	NULL	0	NULL	signs of coronary spasm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of unstable angina with signs of coronary spasm is the least favorable ANO variant in terms of the risk of grave ventricular arrhythmias .
	manualset3
144428	4	409198	5	NULL	NULL	0	NULL	ANO variant	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of unstable angina with signs of coronary spasm is the least favorable ANO variant in terms of the risk of grave ventricular arrhythmias .
	manualset3
144429	5	409198	5	NULL	NULL	0	NULL	risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The combination of unstable angina with signs of coronary spasm is the least favorable ANO variant in terms of the risk of grave ventricular arrhythmias .
	manualset3
144430	6	409198	5	NULL	NULL	NULL	NULL	grave ventricular arrhythmias	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The combination of unstable angina with signs of coronary spasm is the least favorable ANO variant in terms of the risk of grave ventricular arrhythmias .
	manualset3
144431	1	409199	5	NULL	NULL	0	NULL	combinations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The combinations of alpha interferon and 5-FU and of alpha interferon and interleukin-2 ( IL-2 ) are the focus of this paper .
	manualset3
144432	2	409199	5	NULL	NULL	0	NULL	alpha interferon 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The combinations of alpha interferon and 5-FU and of alpha interferon and interleukin-2 ( IL-2 ) are the focus of this paper .
	manualset3
144433	3	409199	5	NULL	NULL	0	NULL	5-FU	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The combinations of alpha interferon and 5-FU and of alpha interferon and interleukin-2 ( IL-2 ) are the focus of this paper .
	manualset3
144434	4	409199	5	NULL	NULL	0	NULL	alpha interferon 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The combinations of alpha interferon and 5-FU and of alpha interferon and interleukin-2 ( IL-2 ) are the focus of this paper .
	manualset3
144435	5	409199	5	NULL	NULL	0	NULL	interleukin-2 ( IL-2 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The combinations of alpha interferon and 5-FU and of alpha interferon and interleukin-2 ( IL-2 ) are the focus of this paper .
	manualset3
144436	6	409199	5	NULL	NULL	0	NULL	focus 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The combinations of alpha interferon and 5-FU and of alpha interferon and interleukin-2 ( IL-2 ) are the focus of this paper .
	manualset3
144437	7	409199	5	NULL	NULL	0	NULL	paper 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The combinations of alpha interferon and 5-FU and of alpha interferon and interleukin-2 ( IL-2 ) are the focus of this paper .
	manualset3
144438	1	409200	5	NULL	NULL	0	NULL	combined in-source decay/post-source decay experiments 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The combined in-source decay/post-source decay experiments revealed the formation of a double bond between C-2 and C-3 in N-acetylglucosamine of Le ( X ) .
	manualset3
144439	2	409200	5	NULL	NULL	0	NULL	formation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The combined in-source decay/post-source decay experiments revealed the formation of a double bond between C-2 and C-3 in N-acetylglucosamine of Le ( X ) .
	manualset3
144440	3	409200	5	NULL	NULL	0	NULL	double bond 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The combined in-source decay/post-source decay experiments revealed the formation of a double bond between C-2 and C-3 in N-acetylglucosamine of Le ( X ) .
	manualset3
144441	4	409200	5	NULL	NULL	0	NULL	C-2	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The combined in-source decay/post-source decay experiments revealed the formation of a double bond between C-2 and C-3 in N-acetylglucosamine of Le ( X ) .
	manualset3
144442	5	409200	5	NULL	NULL	0	NULL	C-3 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The combined in-source decay/post-source decay experiments revealed the formation of a double bond between C-2 and C-3 in N-acetylglucosamine of Le ( X ) .
	manualset3
144443	6	409200	5	NULL	NULL	0	NULL	N-acetylglucosamine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The combined in-source decay/post-source decay experiments revealed the formation of a double bond between C-2 and C-3 in N-acetylglucosamine of Le ( X ) .
	manualset3
144444	7	409200	5	NULL	NULL	0	NULL	Le ( X )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The combined in-source decay/post-source decay experiments revealed the formation of a double bond between C-2 and C-3 in N-acetylglucosamine of Le ( X ) .
	manualset3
144445	1	409201	5	NULL	NULL	0	NULL	combined pharmacological approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The combined pharmacological approach to the treatment of HIV infection , known as highly active antiretroviral therapy ( HAART ) , has dramatically reduced AIDS-related morbidity and mortality .
	manualset3
144446	2	409201	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The combined pharmacological approach to the treatment of HIV infection , known as highly active antiretroviral therapy ( HAART ) , has dramatically reduced AIDS-related morbidity and mortality .
	manualset3
144447	3	409201	5	NULL	NULL	0	NULL	HIV infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The combined pharmacological approach to the treatment of HIV infection , known as highly active antiretroviral therapy ( HAART ) , has dramatically reduced AIDS-related morbidity and mortality .
	manualset3
144448	4	409201	5	NULL	NULL	0	NULL	highly active antiretroviral therapy ( HAART ) 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The combined pharmacological approach to the treatment of HIV infection , known as highly active antiretroviral therapy ( HAART ) , has dramatically reduced AIDS-related morbidity and mortality .
	manualset3
144449	5	409201	5	NULL	NULL	0	NULL	AIDS-related morbidity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The combined pharmacological approach to the treatment of HIV infection , known as highly active antiretroviral therapy ( HAART ) , has dramatically reduced AIDS-related morbidity and mortality .
	manualset3
144450	6	409201	5	NULL	NULL	0	NULL	mortality 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The combined pharmacological approach to the treatment of HIV infection , known as highly active antiretroviral therapy ( HAART ) , has dramatically reduced AIDS-related morbidity and mortality .
	manualset3
144451	1	409202	5	NULL	NULL	0	NULL	combined effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The combined effects of alpha 1-adrenoceptor blockade and 5-HT1A receptor stimulation ( urapidil and 5-methylurapidil ) result in distinct decreases in blood pressure and slight suppression of reflex tachycardia at rest after high doses .
	manualset3
144452	2	409202	5	NULL	NULL	0	NULL	alpha 1-adrenoceptor blockade	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The combined effects of alpha 1-adrenoceptor blockade and 5-HT1A receptor stimulation ( urapidil and 5-methylurapidil ) result in distinct decreases in blood pressure and slight suppression of reflex tachycardia at rest after high doses .
	manualset3
144453	3	409202	5	NULL	NULL	0	NULL	 5-HT1A receptor stimulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The combined effects of alpha 1-adrenoceptor blockade and 5-HT1A receptor stimulation ( urapidil and 5-methylurapidil ) result in distinct decreases in blood pressure and slight suppression of reflex tachycardia at rest after high doses .
	manualset3
144454	4	409202	5	NULL	NULL	0	NULL	urapidil 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The combined effects of alpha 1-adrenoceptor blockade and 5-HT1A receptor stimulation ( urapidil and 5-methylurapidil ) result in distinct decreases in blood pressure and slight suppression of reflex tachycardia at rest after high doses .
	manualset3
144455	5	409202	5	NULL	NULL	0	NULL	5-methylurapidil 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The combined effects of alpha 1-adrenoceptor blockade and 5-HT1A receptor stimulation ( urapidil and 5-methylurapidil ) result in distinct decreases in blood pressure and slight suppression of reflex tachycardia at rest after high doses .
	manualset3
144456	6	409202	5	NULL	NULL	0	NULL	blood pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The combined effects of alpha 1-adrenoceptor blockade and 5-HT1A receptor stimulation ( urapidil and 5-methylurapidil ) result in distinct decreases in blood pressure and slight suppression of reflex tachycardia at rest after high doses .
	manualset3
144457	7	409202	5	NULL	NULL	0	NULL	suppression 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The combined effects of alpha 1-adrenoceptor blockade and 5-HT1A receptor stimulation ( urapidil and 5-methylurapidil ) result in distinct decreases in blood pressure and slight suppression of reflex tachycardia at rest after high doses .
	manualset3
144458	8	409202	5	NULL	NULL	0	NULL	reflex tachycardia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The combined effects of alpha 1-adrenoceptor blockade and 5-HT1A receptor stimulation ( urapidil and 5-methylurapidil ) result in distinct decreases in blood pressure and slight suppression of reflex tachycardia at rest after high doses .
	manualset3
144459	9	409202	5	NULL	NULL	0	NULL	rest 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The combined effects of alpha 1-adrenoceptor blockade and 5-HT1A receptor stimulation ( urapidil and 5-methylurapidil ) result in distinct decreases in blood pressure and slight suppression of reflex tachycardia at rest after high doses .
	manualset3
144460	10	409202	5	NULL	NULL	0	NULL	doses 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The combined effects of alpha 1-adrenoceptor blockade and 5-HT1A receptor stimulation ( urapidil and 5-methylurapidil ) result in distinct decreases in blood pressure and slight suppression of reflex tachycardia at rest after high doses .
	manualset3
144461	1	409203	5	NULL	NULL	0	NULL	correlation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant correlation was also found between AOPP blood levels ratio ( sample B/sample A ) in each baby , and the correspondent level of pain .
	manualset3
144462	2	409203	5	NULL	NULL	0	NULL	AOPP blood levels ratio ( sample B/sample A )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant correlation was also found between AOPP blood levels ratio ( sample B/sample A ) in each baby , and the correspondent level of pain .
	manualset3
144463	3	409203	5	NULL	NULL	0	NULL	baby 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant correlation was also found between AOPP blood levels ratio ( sample B/sample A ) in each baby , and the correspondent level of pain .
	manualset3
144464	4	409203	5	NULL	NULL	0	NULL	correspondent level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant correlation was also found between AOPP blood levels ratio ( sample B/sample A ) in each baby , and the correspondent level of pain .
	manualset3
144465	5	409203	5	NULL	NULL	0	NULL	pain 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant correlation was also found between AOPP blood levels ratio ( sample B/sample A ) in each baby , and the correspondent level of pain .
	manualset3
144466	1	409204	5	NULL	NULL	0	NULL	combined effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The combined effects of the glutamine 64 and phenylalanine 29 in elephant myoglobin largely account for its increased imidazole association and dissociation rate constants , respectively , compared to those of sperm whale myoglobin .
	manualset3
144467	2	409204	5	NULL	NULL	0	NULL	glutamine 64	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The combined effects of the glutamine 64 and phenylalanine 29 in elephant myoglobin largely account for its increased imidazole association and dissociation rate constants , respectively , compared to those of sperm whale myoglobin .
	manualset3
144468	3	409204	5	NULL	NULL	0	NULL	phenylalanine 29 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The combined effects of the glutamine 64 and phenylalanine 29 in elephant myoglobin largely account for its increased imidazole association and dissociation rate constants , respectively , compared to those of sperm whale myoglobin .
	manualset3
144469	4	409204	5	NULL	NULL	0	NULL	elephant myoglobin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The combined effects of the glutamine 64 and phenylalanine 29 in elephant myoglobin largely account for its increased imidazole association and dissociation rate constants , respectively , compared to those of sperm whale myoglobin .
	manualset3
144470	5	409204	5	NULL	NULL	0	NULL	imidazole associationrate constant	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The combined effects of the glutamine 64 and phenylalanine 29 in elephant myoglobin largely account for its increased imidazole association and dissociation rate constants , respectively , compared to those of sperm whale myoglobin .
	manualset3
144471	6	409204	5	NULL	NULL	0	NULL	dissociation rate constant	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The combined effects of the glutamine 64 and phenylalanine 29 in elephant myoglobin largely account for its increased imidazole association and dissociation rate constants , respectively , compared to those of sperm whale myoglobin .
	manualset3
144472	7	409204	5	NULL	NULL	0	NULL	sperm whale myoglobin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The combined effects of the glutamine 64 and phenylalanine 29 in elephant myoglobin largely account for its increased imidazole association and dissociation rate constants , respectively , compared to those of sperm whale myoglobin .
	manualset3
144473	1	409205	5	NULL	NULL	0	NULL	MWCNTs 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The combining of MWCNTs that can hinder the agglomeration and enhance the electronic conductivity of the active materials is responsible for the enhanced cyclic performance .
	manualset3
144474	2	409205	5	NULL	NULL	0	NULL	agglomeration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The combining of MWCNTs that can hinder the agglomeration and enhance the electronic conductivity of the active materials is responsible for the enhanced cyclic performance .
	manualset3
144475	3	409205	5	NULL	NULL	0	NULL	electronic conductivity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The combining of MWCNTs that can hinder the agglomeration and enhance the electronic conductivity of the active materials is responsible for the enhanced cyclic performance .
	manualset3
144476	4	409205	5	NULL	NULL	0	NULL	active materials 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The combining of MWCNTs that can hinder the agglomeration and enhance the electronic conductivity of the active materials is responsible for the enhanced cyclic performance .
	manualset3
144477	5	409205	5	NULL	NULL	0	NULL	enhanced cyclic performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The combining of MWCNTs that can hinder the agglomeration and enhance the electronic conductivity of the active materials is responsible for the enhanced cyclic performance .
	manualset3
144478	1	409206	5	NULL	NULL	0	NULL	common assumption	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The common assumption in quantitative trait locus ( QTL ) linkage mapping studies that parents of multiple connected populations are unrelated is unrealistic for many plant breeding programs .
	manualset3
144479	2	409206	5	NULL	NULL	0	NULL	quantitative trait locus ( QTL ) linkage mapping studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The common assumption in quantitative trait locus ( QTL ) linkage mapping studies that parents of multiple connected populations are unrelated is unrealistic for many plant breeding programs .
	manualset3
144480	3	409206	5	NULL	NULL	NULL	NULL	parents 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The common assumption in quantitative trait locus ( QTL ) linkage mapping studies that parents of multiple connected populations are unrelated is unrealistic for many plant breeding programs .
	manualset3
144481	4	409206	5	NULL	NULL	NULL	NULL	multiple connected populations	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The common assumption in quantitative trait locus ( QTL ) linkage mapping studies that parents of multiple connected populations are unrelated is unrealistic for many plant breeding programs .
	manualset3
144482	5	409206	5	NULL	NULL	0	NULL	plant breeding programs 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The common assumption in quantitative trait locus ( QTL ) linkage mapping studies that parents of multiple connected populations are unrelated is unrealistic for many plant breeding programs .
	manualset3
144483	1	409207	5	NULL	NULL	0	NULL	characteristic structural element 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The common characteristic structural element of cinnamyl phenylpropyl materials is an aryl substituted primary alcohol/aldehyde/ester .
	manualset3
144484	2	409207	5	NULL	NULL	0	NULL	cinnamyl phenylpropyl materials	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The common characteristic structural element of cinnamyl phenylpropyl materials is an aryl substituted primary alcohol/aldehyde/ester .
	manualset3
144485	3	409207	5	NULL	NULL	0	NULL	aryl substituted primary alcohol/aldehyde/ester 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The common characteristic structural element of cinnamyl phenylpropyl materials is an aryl substituted primary alcohol/aldehyde/ester .
	manualset3
144486	1	409208	5	NULL	NULL	0	NULL	commonest complication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The commonest complication of traumatic pancreatitis is the development of pancreatic pseudocyst .
	manualset3
144487	2	409208	5	NULL	NULL	0	NULL	traumatic pancreatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The commonest complication of traumatic pancreatitis is the development of pancreatic pseudocyst .
	manualset3
144488	3	409208	5	NULL	NULL	0	NULL	development of pancreatic pseudocyst	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The commonest complication of traumatic pancreatitis is the development of pancreatic pseudocyst .
	manualset3
144489	1	409209	5	NULL	NULL	0	NULL	companies 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The companies that master the complexity of the ubiquitous Internet will gain significant advantages : they 'll gain greater intimacy with customers and target market segments more efficiently .
	manualset3
144490	2	409209	5	NULL	NULL	0	NULL	complexity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The companies that master the complexity of the ubiquitous Internet will gain significant advantages : they 'll gain greater intimacy with customers and target market segments more efficiently .
	manualset3
144491	3	409209	5	NULL	NULL	0	NULL	ubiquitous Internet	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The companies that master the complexity of the ubiquitous Internet will gain significant advantages : they 'll gain greater intimacy with customers and target market segments more efficiently .
	manualset3
144492	4	409209	5	NULL	NULL	0	NULL	significant advantages 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The companies that master the complexity of the ubiquitous Internet will gain significant advantages : they 'll gain greater intimacy with customers and target market segments more efficiently .
	manualset3
144493	5	409209	5	NULL	NULL	0	NULL	intimacy 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The companies that master the complexity of the ubiquitous Internet will gain significant advantages : they 'll gain greater intimacy with customers and target market segments more efficiently .
	manualset3
144494	6	409209	5	NULL	NULL	0	NULL	customers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The companies that master the complexity of the ubiquitous Internet will gain significant advantages : they 'll gain greater intimacy with customers and target market segments more efficiently .
	manualset3
144495	7	409209	5	NULL	NULL	0	NULL	target market segments	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The companies that master the complexity of the ubiquitous Internet will gain significant advantages : they 'll gain greater intimacy with customers and target market segments more efficiently .
	manualset3
144496	1	409210	5	NULL	NULL	0	NULL	company 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The company has reported that phase III trials will begin by the end of 2000 .
	manualset3
144497	2	409210	5	NULL	NULL	0	NULL	phase III trials 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The company has reported that phase III trials will begin by the end of 2000 .
	manualset3
144498	3	409210	5	NULL	NULL	0	NULL	2000 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	The company has reported that phase III trials will begin by the end of 2000 .
	manualset3
144499	1	409211	5	NULL	NULL	0	NULL	comparative effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative effects of 10 different dietary fibers on serum and liver lipids were investigated by feeding male Sprague-Dawley rats diets containing 10 g cholesterol + 2 g cholic acid/kg diet , with 60 g fiber/kg diet .
	manualset3
144500	2	409211	5	NULL	NULL	0	NULL	10	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative effects of 10 different dietary fibers on serum and liver lipids were investigated by feeding male Sprague-Dawley rats diets containing 10 g cholesterol + 2 g cholic acid/kg diet , with 60 g fiber/kg diet .
	manualset3
144501	3	409211	5	NULL	NULL	0	NULL	dietary fibers	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative effects of 10 different dietary fibers on serum and liver lipids were investigated by feeding male Sprague-Dawley rats diets containing 10 g cholesterol + 2 g cholic acid/kg diet , with 60 g fiber/kg diet .
	manualset3
144502	4	409211	5	NULL	NULL	0	NULL	serum 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative effects of 10 different dietary fibers on serum and liver lipids were investigated by feeding male Sprague-Dawley rats diets containing 10 g cholesterol + 2 g cholic acid/kg diet , with 60 g fiber/kg diet .
	manualset3
144503	5	409211	5	NULL	NULL	0	NULL	liver lipids	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative effects of 10 different dietary fibers on serum and liver lipids were investigated by feeding male Sprague-Dawley rats diets containing 10 g cholesterol + 2 g cholic acid/kg diet , with 60 g fiber/kg diet .
	manualset3
144504	6	409211	5	NULL	NULL	0	NULL	male Sprague-Dawley rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative effects of 10 different dietary fibers on serum and liver lipids were investigated by feeding male Sprague-Dawley rats diets containing 10 g cholesterol + 2 g cholic acid/kg diet , with 60 g fiber/kg diet .
	manualset3
144505	7	409211	5	NULL	NULL	0	NULL	diets 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative effects of 10 different dietary fibers on serum and liver lipids were investigated by feeding male Sprague-Dawley rats diets containing 10 g cholesterol + 2 g cholic acid/kg diet , with 60 g fiber/kg diet .
	manualset3
144506	8	409211	5	NULL	NULL	0	NULL	10 g cholesterol + 2 g cholic acid/kg diet 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative effects of 10 different dietary fibers on serum and liver lipids were investigated by feeding male Sprague-Dawley rats diets containing 10 g cholesterol + 2 g cholic acid/kg diet , with 60 g fiber/kg diet .
	manualset3
144507	9	409211	5	NULL	NULL	0	NULL	60 g fiber/kg diet	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative effects of 10 different dietary fibers on serum and liver lipids were investigated by feeding male Sprague-Dawley rats diets containing 10 g cholesterol + 2 g cholic acid/kg diet , with 60 g fiber/kg diet .
	manualset3
144508	1	409212	5	NULL	NULL	0	NULL	depletion 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant depletion of the neuropeptides was found in the region of the wound within two days , and this persisted for two weeks .
	manualset3
144509	2	409212	5	NULL	NULL	0	NULL	neuropeptides 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant depletion of the neuropeptides was found in the region of the wound within two days , and this persisted for two weeks .
	manualset3
144510	3	409212	5	NULL	NULL	0	NULL	region of the wound	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant depletion of the neuropeptides was found in the region of the wound within two days , and this persisted for two weeks .
	manualset3
144511	4	409212	5	NULL	NULL	0	NULL	two days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant depletion of the neuropeptides was found in the region of the wound within two days , and this persisted for two weeks .
	manualset3
144512	5	409212	5	NULL	NULL	0	NULL	two weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant depletion of the neuropeptides was found in the region of the wound within two days , and this persisted for two weeks .
	manualset3
144513	1	409213	5	NULL	NULL	0	NULL	comparative microspectrophotometric study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative microspectrophotometric study of the DNA content in histological samples of 5 pigmented nevi , 3 dysplastic , 9 pigmented nevi with traits of malignization , and 10 malignant melanomas with the I-V invasion level by Clark has permitted determining a direct relationship between the expression degree and quality of the proliferation processes in neoplasia , on the one hand , and DNA quantity in nuclei , on the other hand .
	manualset3
144514	2	409213	5	NULL	NULL	0	NULL	DNA content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative microspectrophotometric study of the DNA content in histological samples of 5 pigmented nevi , 3 dysplastic , 9 pigmented nevi with traits of malignization , and 10 malignant melanomas with the I-V invasion level by Clark has permitted determining a direct relationship between the expression degree and quality of the proliferation processes in neoplasia , on the one hand , and DNA quantity in nuclei , on the other hand .
	manualset3
144515	3	409213	5	NULL	NULL	0	NULL	histological samples	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative microspectrophotometric study of the DNA content in histological samples of 5 pigmented nevi , 3 dysplastic , 9 pigmented nevi with traits of malignization , and 10 malignant melanomas with the I-V invasion level by Clark has permitted determining a direct relationship between the expression degree and quality of the proliferation processes in neoplasia , on the one hand , and DNA quantity in nuclei , on the other hand .
	manualset3
144516	4	409213	5	NULL	NULL	0	NULL	5 pigmented nevi 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative microspectrophotometric study of the DNA content in histological samples of 5 pigmented nevi , 3 dysplastic , 9 pigmented nevi with traits of malignization , and 10 malignant melanomas with the I-V invasion level by Clark has permitted determining a direct relationship between the expression degree and quality of the proliferation processes in neoplasia , on the one hand , and DNA quantity in nuclei , on the other hand .
	manualset3
144517	5	409213	5	NULL	NULL	0	NULL	3 dysplastic	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative microspectrophotometric study of the DNA content in histological samples of 5 pigmented nevi , 3 dysplastic , 9 pigmented nevi with traits of malignization , and 10 malignant melanomas with the I-V invasion level by Clark has permitted determining a direct relationship between the expression degree and quality of the proliferation processes in neoplasia , on the one hand , and DNA quantity in nuclei , on the other hand .
	manualset3
144518	6	409213	5	NULL	NULL	0	NULL	9 pigmented nevi 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative microspectrophotometric study of the DNA content in histological samples of 5 pigmented nevi , 3 dysplastic , 9 pigmented nevi with traits of malignization , and 10 malignant melanomas with the I-V invasion level by Clark has permitted determining a direct relationship between the expression degree and quality of the proliferation processes in neoplasia , on the one hand , and DNA quantity in nuclei , on the other hand .
	manualset3
144519	7	409213	5	NULL	NULL	0	NULL	traits of malignization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative microspectrophotometric study of the DNA content in histological samples of 5 pigmented nevi , 3 dysplastic , 9 pigmented nevi with traits of malignization , and 10 malignant melanomas with the I-V invasion level by Clark has permitted determining a direct relationship between the expression degree and quality of the proliferation processes in neoplasia , on the one hand , and DNA quantity in nuclei , on the other hand .
	manualset3
144520	8	409213	5	NULL	NULL	0	NULL	10 malignant melanomas	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative microspectrophotometric study of the DNA content in histological samples of 5 pigmented nevi , 3 dysplastic , 9 pigmented nevi with traits of malignization , and 10 malignant melanomas with the I-V invasion level by Clark has permitted determining a direct relationship between the expression degree and quality of the proliferation processes in neoplasia , on the one hand , and DNA quantity in nuclei , on the other hand .
	manualset3
144521	9	409213	5	NULL	NULL	0	NULL	I-V invasion level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative microspectrophotometric study of the DNA content in histological samples of 5 pigmented nevi , 3 dysplastic , 9 pigmented nevi with traits of malignization , and 10 malignant melanomas with the I-V invasion level by Clark has permitted determining a direct relationship between the expression degree and quality of the proliferation processes in neoplasia , on the one hand , and DNA quantity in nuclei , on the other hand .
	manualset3
144522	10	409213	5	NULL	NULL	0	NULL	Clark 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative microspectrophotometric study of the DNA content in histological samples of 5 pigmented nevi , 3 dysplastic , 9 pigmented nevi with traits of malignization , and 10 malignant melanomas with the I-V invasion level by Clark has permitted determining a direct relationship between the expression degree and quality of the proliferation processes in neoplasia , on the one hand , and DNA quantity in nuclei , on the other hand .
	manualset3
144523	11	409213	5	NULL	NULL	0	NULL	relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative microspectrophotometric study of the DNA content in histological samples of 5 pigmented nevi , 3 dysplastic , 9 pigmented nevi with traits of malignization , and 10 malignant melanomas with the I-V invasion level by Clark has permitted determining a direct relationship between the expression degree and quality of the proliferation processes in neoplasia , on the one hand , and DNA quantity in nuclei , on the other hand .
	manualset3
144524	12	409213	5	NULL	NULL	0	NULL	expression degree	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative microspectrophotometric study of the DNA content in histological samples of 5 pigmented nevi , 3 dysplastic , 9 pigmented nevi with traits of malignization , and 10 malignant melanomas with the I-V invasion level by Clark has permitted determining a direct relationship between the expression degree and quality of the proliferation processes in neoplasia , on the one hand , and DNA quantity in nuclei , on the other hand .
	manualset3
144525	13	409213	5	NULL	NULL	0	NULL	quality 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative microspectrophotometric study of the DNA content in histological samples of 5 pigmented nevi , 3 dysplastic , 9 pigmented nevi with traits of malignization , and 10 malignant melanomas with the I-V invasion level by Clark has permitted determining a direct relationship between the expression degree and quality of the proliferation processes in neoplasia , on the one hand , and DNA quantity in nuclei , on the other hand .
	manualset3
144526	14	409213	5	NULL	NULL	0	NULL	proliferation processes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative microspectrophotometric study of the DNA content in histological samples of 5 pigmented nevi , 3 dysplastic , 9 pigmented nevi with traits of malignization , and 10 malignant melanomas with the I-V invasion level by Clark has permitted determining a direct relationship between the expression degree and quality of the proliferation processes in neoplasia , on the one hand , and DNA quantity in nuclei , on the other hand .
	manualset3
144527	15	409213	5	NULL	NULL	0	NULL	neoplasia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative microspectrophotometric study of the DNA content in histological samples of 5 pigmented nevi , 3 dysplastic , 9 pigmented nevi with traits of malignization , and 10 malignant melanomas with the I-V invasion level by Clark has permitted determining a direct relationship between the expression degree and quality of the proliferation processes in neoplasia , on the one hand , and DNA quantity in nuclei , on the other hand .
	manualset3
144528	16	409213	5	NULL	NULL	0	NULL	DNA quantity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative microspectrophotometric study of the DNA content in histological samples of 5 pigmented nevi , 3 dysplastic , 9 pigmented nevi with traits of malignization , and 10 malignant melanomas with the I-V invasion level by Clark has permitted determining a direct relationship between the expression degree and quality of the proliferation processes in neoplasia , on the one hand , and DNA quantity in nuclei , on the other hand .
	manualset3
144529	17	409213	5	NULL	NULL	0	NULL	nuclei 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative microspectrophotometric study of the DNA content in histological samples of 5 pigmented nevi , 3 dysplastic , 9 pigmented nevi with traits of malignization , and 10 malignant melanomas with the I-V invasion level by Clark has permitted determining a direct relationship between the expression degree and quality of the proliferation processes in neoplasia , on the one hand , and DNA quantity in nuclei , on the other hand .
	manualset3
144530	1	409214	5	NULL	NULL	0	NULL	compared analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The compared analysis of PM-MTH produced by microfluidic and conventional bulk mixing procedures revealed that microfluidics provides a useful platform for the production of PM-MTH with improved controllability , reproducibility , smaller size , and polydispersity .
	manualset3
144531	2	409214	5	NULL	NULL	0	NULL	PM-MTH 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The compared analysis of PM-MTH produced by microfluidic and conventional bulk mixing procedures revealed that microfluidics provides a useful platform for the production of PM-MTH with improved controllability , reproducibility , smaller size , and polydispersity .
	manualset3
144532	3	409214	5	NULL	NULL	0	NULL	microfluidic and conventional bulk mixing procedures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The compared analysis of PM-MTH produced by microfluidic and conventional bulk mixing procedures revealed that microfluidics provides a useful platform for the production of PM-MTH with improved controllability , reproducibility , smaller size , and polydispersity .
	manualset3
144533	4	409214	5	NULL	NULL	0	NULL	microfluidics 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The compared analysis of PM-MTH produced by microfluidic and conventional bulk mixing procedures revealed that microfluidics provides a useful platform for the production of PM-MTH with improved controllability , reproducibility , smaller size , and polydispersity .
	manualset3
144534	5	409214	5	NULL	NULL	0	NULL	platform 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The compared analysis of PM-MTH produced by microfluidic and conventional bulk mixing procedures revealed that microfluidics provides a useful platform for the production of PM-MTH with improved controllability , reproducibility , smaller size , and polydispersity .
	manualset3
144535	6	409214	5	NULL	NULL	0	NULL	production 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The compared analysis of PM-MTH produced by microfluidic and conventional bulk mixing procedures revealed that microfluidics provides a useful platform for the production of PM-MTH with improved controllability , reproducibility , smaller size , and polydispersity .
	manualset3
144536	7	409214	5	NULL	NULL	0	NULL	PM-MTH 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The compared analysis of PM-MTH produced by microfluidic and conventional bulk mixing procedures revealed that microfluidics provides a useful platform for the production of PM-MTH with improved controllability , reproducibility , smaller size , and polydispersity .
	manualset3
144537	8	409214	5	NULL	NULL	NULL	NULL	controllability 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The compared analysis of PM-MTH produced by microfluidic and conventional bulk mixing procedures revealed that microfluidics provides a useful platform for the production of PM-MTH with improved controllability , reproducibility , smaller size , and polydispersity .
	manualset3
144538	9	409214	5	NULL	NULL	0	NULL	reproducibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The compared analysis of PM-MTH produced by microfluidic and conventional bulk mixing procedures revealed that microfluidics provides a useful platform for the production of PM-MTH with improved controllability , reproducibility , smaller size , and polydispersity .
	manualset3
144539	10	409214	5	NULL	NULL	0	NULL	size 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The compared analysis of PM-MTH produced by microfluidic and conventional bulk mixing procedures revealed that microfluidics provides a useful platform for the production of PM-MTH with improved controllability , reproducibility , smaller size , and polydispersity .
	manualset3
144540	11	409214	5	NULL	NULL	0	NULL	polydispersity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The compared analysis of PM-MTH produced by microfluidic and conventional bulk mixing procedures revealed that microfluidics provides a useful platform for the production of PM-MTH with improved controllability , reproducibility , smaller size , and polydispersity .
	manualset3
144541	1	409215	5	NULL	NULL	0	NULL	comparison 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparison of estimated values with W.H.O drinking water standards revealed that water of the study area is polluted with reference to a number of physico-chemical parameters studied .
	manualset3
144542	2	409215	5	NULL	NULL	0	NULL	estimated values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparison of estimated values with W.H.O drinking water standards revealed that water of the study area is polluted with reference to a number of physico-chemical parameters studied .
	manualset3
144543	3	409215	5	NULL	NULL	0	NULL	W.H.O drinking water standards 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparison of estimated values with W.H.O drinking water standards revealed that water of the study area is polluted with reference to a number of physico-chemical parameters studied .
	manualset3
144544	4	409215	5	NULL	NULL	0	NULL	water 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparison of estimated values with W.H.O drinking water standards revealed that water of the study area is polluted with reference to a number of physico-chemical parameters studied .
	manualset3
144545	5	409215	5	NULL	NULL	0	NULL	study area	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparison of estimated values with W.H.O drinking water standards revealed that water of the study area is polluted with reference to a number of physico-chemical parameters studied .
	manualset3
144546	6	409215	5	NULL	NULL	0	NULL	reference 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparison of estimated values with W.H.O drinking water standards revealed that water of the study area is polluted with reference to a number of physico-chemical parameters studied .
	manualset3
144547	7	409215	5	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparison of estimated values with W.H.O drinking water standards revealed that water of the study area is polluted with reference to a number of physico-chemical parameters studied .
	manualset3
144548	8	409215	5	NULL	NULL	0	NULL	physico-chemical parameters	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparison of estimated values with W.H.O drinking water standards revealed that water of the study area is polluted with reference to a number of physico-chemical parameters studied .
	manualset3
144549	1	409216	5	NULL	NULL	0	NULL	comparison 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparison of methods suggested that the cloning , cultivation , and quantitative PCR methods complemented each other , generating a more comprehensive picture of fungal flora than any of the methods would give alone .
	manualset3
144550	2	409216	5	NULL	NULL	0	NULL	methods 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparison of methods suggested that the cloning , cultivation , and quantitative PCR methods complemented each other , generating a more comprehensive picture of fungal flora than any of the methods would give alone .
	manualset3
144551	3	409216	5	NULL	NULL	0	NULL	cloning 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparison of methods suggested that the cloning , cultivation , and quantitative PCR methods complemented each other , generating a more comprehensive picture of fungal flora than any of the methods would give alone .
	manualset3
144552	4	409216	5	NULL	NULL	0	NULL	cultivation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparison of methods suggested that the cloning , cultivation , and quantitative PCR methods complemented each other , generating a more comprehensive picture of fungal flora than any of the methods would give alone .
	manualset3
144553	5	409216	5	NULL	NULL	0	NULL	quantitative PCR methods 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparison of methods suggested that the cloning , cultivation , and quantitative PCR methods complemented each other , generating a more comprehensive picture of fungal flora than any of the methods would give alone .
	manualset3
144554	6	409216	5	NULL	NULL	0	NULL	comprehensive picture	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparison of methods suggested that the cloning , cultivation , and quantitative PCR methods complemented each other , generating a more comprehensive picture of fungal flora than any of the methods would give alone .
	manualset3
144555	7	409216	5	NULL	NULL	0	NULL	fungal flora	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparison of methods suggested that the cloning , cultivation , and quantitative PCR methods complemented each other , generating a more comprehensive picture of fungal flora than any of the methods would give alone .
	manualset3
144556	8	409216	5	NULL	NULL	0	NULL	methods 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparison of methods suggested that the cloning , cultivation , and quantitative PCR methods complemented each other , generating a more comprehensive picture of fungal flora than any of the methods would give alone .
	manualset3
144557	1	409217	5	NULL	NULL	0	NULL	comparison 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparison of theoretically calculated and experimentally determined yield for Lu176 ( n , gamma ) Lu177 reaction is presented .
	manualset3
144558	2	409217	5	NULL	NULL	0	NULL	theoretically calculated yield	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparison of theoretically calculated and experimentally determined yield for Lu176 ( n , gamma ) Lu177 reaction is presented .
	manualset3
144559	3	409217	5	NULL	NULL	0	NULL	experimentally determined yield	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparison of theoretically calculated and experimentally determined yield for Lu176 ( n , gamma ) Lu177 reaction is presented .
	manualset3
144560	4	409217	5	NULL	NULL	0	NULL	Lu176 ( n , gamma ) Lu177 reaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparison of theoretically calculated and experimentally determined yield for Lu176 ( n , gamma ) Lu177 reaction is presented .
	manualset3
144561	1	409218	5	NULL	NULL	0	NULL	competition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The competition between the growth of the facets protected by imidazole and Ag controls the morphology transformation via truncation of octahedrons at vertices or edges .
	manualset3
144562	2	409218	5	NULL	NULL	0	NULL	growth 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The competition between the growth of the facets protected by imidazole and Ag controls the morphology transformation via truncation of octahedrons at vertices or edges .
	manualset3
144563	3	409218	5	NULL	NULL	0	NULL	facets 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The competition between the growth of the facets protected by imidazole and Ag controls the morphology transformation via truncation of octahedrons at vertices or edges .
	manualset3
144564	4	409218	5	NULL	NULL	0	NULL	imidazole 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The competition between the growth of the facets protected by imidazole and Ag controls the morphology transformation via truncation of octahedrons at vertices or edges .
	manualset3
144565	5	409218	5	NULL	NULL	0	NULL	Ag	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The competition between the growth of the facets protected by imidazole and Ag controls the morphology transformation via truncation of octahedrons at vertices or edges .
	manualset3
144566	6	409218	5	NULL	NULL	0	NULL	morphology transformation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The competition between the growth of the facets protected by imidazole and Ag controls the morphology transformation via truncation of octahedrons at vertices or edges .
	manualset3
144567	7	409218	5	NULL	NULL	0	NULL	truncation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The competition between the growth of the facets protected by imidazole and Ag controls the morphology transformation via truncation of octahedrons at vertices or edges .
	manualset3
144568	8	409218	5	NULL	NULL	0	NULL	octahedrons 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The competition between the growth of the facets protected by imidazole and Ag controls the morphology transformation via truncation of octahedrons at vertices or edges .
	manualset3
144569	9	409218	5	NULL	NULL	0	NULL	vertices or edges 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The competition between the growth of the facets protected by imidazole and Ag controls the morphology transformation via truncation of octahedrons at vertices or edges .
	manualset3
144570	1	409219	5	NULL	NULL	0	NULL	competitions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The competitions induced significant increases in RBC , Hb , PCV , MCV and TPP .
	manualset3
144571	2	409219	5	NULL	NULL	0	NULL	RBC 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The competitions induced significant increases in RBC , Hb , PCV , MCV and TPP .
	manualset3
144572	3	409219	5	NULL	NULL	0	NULL	Hb 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The competitions induced significant increases in RBC , Hb , PCV , MCV and TPP .
	manualset3
144573	4	409219	5	NULL	NULL	0	NULL	PCV 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The competitions induced significant increases in RBC , Hb , PCV , MCV and TPP .
	manualset3
144574	5	409219	5	NULL	NULL	0	NULL	MCV 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The competitions induced significant increases in RBC , Hb , PCV , MCV and TPP .
	manualset3
144575	6	409219	5	NULL	NULL	0	NULL	TPP 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The competitions induced significant increases in RBC , Hb , PCV , MCV and TPP .
	manualset3
144576	1	409220	5	NULL	NULL	0	NULL	complement-dependent bactericidal activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The complement-dependent bactericidal activity of normal nasal airway surface fluid and sputum against ChoP-expressing H. influenzae was abolished when the secretions were pretreated to remove CRP .
	manualset3
144577	2	409220	5	NULL	NULL	0	NULL	normal nasal airway surface fluid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The complement-dependent bactericidal activity of normal nasal airway surface fluid and sputum against ChoP-expressing H. influenzae was abolished when the secretions were pretreated to remove CRP .
	manualset3
144578	3	409220	5	NULL	NULL	0	NULL	sputum 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The complement-dependent bactericidal activity of normal nasal airway surface fluid and sputum against ChoP-expressing H. influenzae was abolished when the secretions were pretreated to remove CRP .
	manualset3
144579	4	409220	5	NULL	NULL	0	NULL	ChoP-expressing H. influenzae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The complement-dependent bactericidal activity of normal nasal airway surface fluid and sputum against ChoP-expressing H. influenzae was abolished when the secretions were pretreated to remove CRP .
	manualset3
144580	5	409220	5	NULL	NULL	0	NULL	secretions 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The complement-dependent bactericidal activity of normal nasal airway surface fluid and sputum against ChoP-expressing H. influenzae was abolished when the secretions were pretreated to remove CRP .
	manualset3
144581	6	409220	5	NULL	NULL	0	NULL	CRP 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The complement-dependent bactericidal activity of normal nasal airway surface fluid and sputum against ChoP-expressing H. influenzae was abolished when the secretions were pretreated to remove CRP .
	manualset3
144582	1	409221	5	NULL	NULL	0	NULL	complement system	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The complement system in bullous pemphigoid .
	manualset3
144583	2	409221	5	NULL	NULL	0	NULL	bullous pemphigoid	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The complement system in bullous pemphigoid .
	manualset3
144584	1	409222	5	NULL	NULL	0	NULL	complementary DNAs 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The complementary DNAs for both the chicken cEryf 1 ( ref .
	manualset3
144585	2	409222	5	NULL	NULL	0	NULL	chicken cEryf 1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The complementary DNAs for both the chicken cEryf 1 ( ref .
	manualset3
144586	1	409223	5	NULL	NULL	0	NULL	complete 1H NMR assignments	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The complete 1H NMR assignments for momilactone A and B and 13C NMR assignments for tricin are discussed .
	manualset3
144587	2	409223	5	NULL	NULL	0	NULL	momilactone A	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The complete 1H NMR assignments for momilactone A and B and 13C NMR assignments for tricin are discussed .
	manualset3
144588	3	409223	5	NULL	NULL	0	NULL	momilactone B	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The complete 1H NMR assignments for momilactone A and B and 13C NMR assignments for tricin are discussed .
	manualset3
144589	4	409223	5	NULL	NULL	0	NULL	13C NMR assignments	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The complete 1H NMR assignments for momilactone A and B and 13C NMR assignments for tricin are discussed .
	manualset3
144590	5	409223	5	NULL	NULL	0	NULL	tricin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The complete 1H NMR assignments for momilactone A and B and 13C NMR assignments for tricin are discussed .
	manualset3
144591	1	409224	5	NULL	NULL	0	NULL	complete blood count 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The complete blood count and leukocyte differential count have no value in screening asymptomatic members of the general population .
	manualset3
144592	2	409224	5	NULL	NULL	0	NULL	leukocyte differential count 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The complete blood count and leukocyte differential count have no value in screening asymptomatic members of the general population .
	manualset3
144593	3	409224	5	NULL	NULL	0	NULL	value 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The complete blood count and leukocyte differential count have no value in screening asymptomatic members of the general population .
	manualset3
144594	4	409224	5	NULL	NULL	0	NULL	asymptomatic members 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The complete blood count and leukocyte differential count have no value in screening asymptomatic members of the general population .
	manualset3
144595	5	409224	5	NULL	NULL	0	NULL	general population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The complete blood count and leukocyte differential count have no value in screening asymptomatic members of the general population .
	manualset3
144596	1	409225	5	NULL	NULL	0	NULL	complete mitochondrial genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The complete mitochondrial genome of the alligator , Alligator mississippiensis , was sequenced .
	manualset3
144597	2	409225	5	NULL	NULL	0	NULL	alligator , Alligator mississippiensis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The complete mitochondrial genome of the alligator , Alligator mississippiensis , was sequenced .
	manualset3
144598	1	409226	5	NULL	NULL	0	NULL	complete normalization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The complete normalization of serum transaminases and bilirubin occurred on average after 5.5 weeks and 3 weeks respectively .
	manualset3
144599	2	409226	5	NULL	NULL	0	NULL	serum transaminases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The complete normalization of serum transaminases and bilirubin occurred on average after 5.5 weeks and 3 weeks respectively .
	manualset3
144600	3	409226	5	NULL	NULL	0	NULL	bilirubin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The complete normalization of serum transaminases and bilirubin occurred on average after 5.5 weeks and 3 weeks respectively .
	manualset3
144601	4	409226	5	NULL	NULL	0	NULL	average 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The complete normalization of serum transaminases and bilirubin occurred on average after 5.5 weeks and 3 weeks respectively .
	manualset3
144602	5	409226	5	NULL	NULL	0	NULL	 5.5 weeks 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The complete normalization of serum transaminases and bilirubin occurred on average after 5.5 weeks and 3 weeks respectively .
	manualset3
144603	6	409226	5	NULL	NULL	0	NULL	3 weeks 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The complete normalization of serum transaminases and bilirubin occurred on average after 5.5 weeks and 3 weeks respectively .
	manualset3
144604	1	409227	5	NULL	NULL	0	NULL	complete sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The complete sequence of orange homologous capsanthin/capsorubin synthase gene is 3788 bp long with a coding sequence of 1512 bp , which encodes a polypeptide of 503 amino acids .
	manualset3
144605	2	409227	5	NULL	NULL	0	NULL	orange homologous capsanthin/capsorubin synthase gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The complete sequence of orange homologous capsanthin/capsorubin synthase gene is 3788 bp long with a coding sequence of 1512 bp , which encodes a polypeptide of 503 amino acids .
	manualset3
144606	3	409227	5	NULL	NULL	0	NULL	3788 bp	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The complete sequence of orange homologous capsanthin/capsorubin synthase gene is 3788 bp long with a coding sequence of 1512 bp , which encodes a polypeptide of 503 amino acids .
	manualset3
144607	4	409227	5	NULL	NULL	0	NULL	coding sequence 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The complete sequence of orange homologous capsanthin/capsorubin synthase gene is 3788 bp long with a coding sequence of 1512 bp , which encodes a polypeptide of 503 amino acids .
	manualset3
144608	5	409227	5	NULL	NULL	0	NULL	1512 bp	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The complete sequence of orange homologous capsanthin/capsorubin synthase gene is 3788 bp long with a coding sequence of 1512 bp , which encodes a polypeptide of 503 amino acids .
	manualset3
144609	6	409227	5	NULL	NULL	0	NULL	polypeptide 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The complete sequence of orange homologous capsanthin/capsorubin synthase gene is 3788 bp long with a coding sequence of 1512 bp , which encodes a polypeptide of 503 amino acids .
	manualset3
144610	7	409227	5	NULL	NULL	0	NULL	503 amino acids	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The complete sequence of orange homologous capsanthin/capsorubin synthase gene is 3788 bp long with a coding sequence of 1512 bp , which encodes a polypeptide of 503 amino acids .
	manualset3
144611	1	409228	5	NULL	NULL	0	NULL	complex structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The complex structure of both the spicule and spicular sheath is unique among all capillariids parasitizing cold-blooded vertebrates .
	manualset3
144612	2	409228	5	NULL	NULL	0	NULL	spicule 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The complex structure of both the spicule and spicular sheath is unique among all capillariids parasitizing cold-blooded vertebrates .
	manualset3
144613	3	409228	5	NULL	NULL	0	NULL	spicular sheath	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The complex structure of both the spicule and spicular sheath is unique among all capillariids parasitizing cold-blooded vertebrates .
	manualset3
144614	4	409228	5	NULL	NULL	0	NULL	capillariids 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The complex structure of both the spicule and spicular sheath is unique among all capillariids parasitizing cold-blooded vertebrates .
	manualset3
144615	5	409228	5	NULL	NULL	0	NULL	cold-blooded vertebrates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The complex structure of both the spicule and spicular sheath is unique among all capillariids parasitizing cold-blooded vertebrates .
	manualset3
144616	1	409229	5	NULL	NULL	0	NULL	complexes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The complexes have intramolecular H-bonds from the urea cavity of ( H31 ) ( 3 - ) to the coordinated hydroxo oxygen .
	manualset3
144617	2	409229	5	NULL	NULL	0	NULL	intramolecular H-bonds	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The complexes have intramolecular H-bonds from the urea cavity of ( H31 ) ( 3 - ) to the coordinated hydroxo oxygen .
	manualset3
144618	3	409229	5	NULL	NULL	0	NULL	urea cavity	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The complexes have intramolecular H-bonds from the urea cavity of ( H31 ) ( 3 - ) to the coordinated hydroxo oxygen .
	manualset3
144619	4	409229	5	NULL	NULL	0	NULL	 ( H31 ) ( 3 - ) 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The complexes have intramolecular H-bonds from the urea cavity of ( H31 ) ( 3 - ) to the coordinated hydroxo oxygen .
	manualset3
144620	5	409229	5	NULL	NULL	NULL	NULL	hydroxo oxygen	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The complexes have intramolecular H-bonds from the urea cavity of ( H31 ) ( 3 - ) to the coordinated hydroxo oxygen .
	manualset3
144621	1	409230	5	NULL	NULL	0	NULL	significant direct correlation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant direct correlation was also detected between the MAGE-A4 / LAGE1 and MAGE-A4 / NY-ESO1 levels of gene expression .
	manualset3
144622	2	409230	5	NULL	NULL	0	NULL	 MAGE-A4 / LAGE1 levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant direct correlation was also detected between the MAGE-A4 / LAGE1 and MAGE-A4 / NY-ESO1 levels of gene expression .
	manualset3
144623	3	409230	5	NULL	NULL	0	NULL	MAGE-A4 / NY-ESO1 levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant direct correlation was also detected between the MAGE-A4 / LAGE1 and MAGE-A4 / NY-ESO1 levels of gene expression .
	manualset3
144624	4	409230	5	NULL	NULL	0	NULL	gene expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant direct correlation was also detected between the MAGE-A4 / LAGE1 and MAGE-A4 / NY-ESO1 levels of gene expression .
	manualset3
144625	1	409231	5	NULL	NULL	0	NULL	components 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The components of this system , with the exception of hydrogen peroxide , are present in milk .
	manualset3
144626	2	409231	5	NULL	NULL	0	NULL	system 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The components of this system , with the exception of hydrogen peroxide , are present in milk .
	manualset3
144627	3	409231	5	NULL	NULL	0	NULL	exception 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The components of this system , with the exception of hydrogen peroxide , are present in milk .
	manualset3
144628	4	409231	5	NULL	NULL	0	NULL	hydrogen peroxide	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The components of this system , with the exception of hydrogen peroxide , are present in milk .
	manualset3
144629	5	409231	5	NULL	NULL	0	NULL	milk 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The components of this system , with the exception of hydrogen peroxide , are present in milk .
	manualset3
144630	1	409232	5	NULL	NULL	0	NULL	composite origin	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The composite origin of the i2 may be associated with its developmental vulnerability .
	manualset3
144631	2	409232	5	NULL	NULL	0	NULL	i2	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The composite origin of the i2 may be associated with its developmental vulnerability .
	manualset3
144632	3	409232	5	NULL	NULL	0	NULL	developmental vulnerability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The composite origin of the i2 may be associated with its developmental vulnerability .
	manualset3
144633	1	409233	5	NULL	NULL	0	NULL	composition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The composition and structure of lignified walls has a dramatic impact on the technological value of raw materials .
	manualset3
144634	2	409233	5	NULL	NULL	0	NULL	structure 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The composition and structure of lignified walls has a dramatic impact on the technological value of raw materials .
	manualset3
144635	3	409233	5	NULL	NULL	NULL	NULL	lignified walls	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The composition and structure of lignified walls has a dramatic impact on the technological value of raw materials .
	manualset3
144636	4	409233	5	NULL	NULL	0	NULL	impact 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The composition and structure of lignified walls has a dramatic impact on the technological value of raw materials .
	manualset3
144637	5	409233	5	NULL	NULL	0	NULL	technological value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The composition and structure of lignified walls has a dramatic impact on the technological value of raw materials .
	manualset3
144638	6	409233	5	NULL	NULL	0	NULL	raw materials	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The composition and structure of lignified walls has a dramatic impact on the technological value of raw materials .
	manualset3
144639	1	409234	5	NULL	NULL	0	NULL	compound 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The compound , showing structural similarities to both phenytoin and dopamine , was found to decrease spontaneous motor activity of mice and to exert a pronounced protective effect against convulsive seizures induced by pentylenetetrazol ( Metrazol ) .
	manualset3
144640	2	409234	5	NULL	NULL	0	NULL	structural similarities 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The compound , showing structural similarities to both phenytoin and dopamine , was found to decrease spontaneous motor activity of mice and to exert a pronounced protective effect against convulsive seizures induced by pentylenetetrazol ( Metrazol ) .
	manualset3
144641	3	409234	5	NULL	NULL	0	NULL	phenytoin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The compound , showing structural similarities to both phenytoin and dopamine , was found to decrease spontaneous motor activity of mice and to exert a pronounced protective effect against convulsive seizures induced by pentylenetetrazol ( Metrazol ) .
	manualset3
144642	4	409234	5	NULL	NULL	0	NULL	dopamine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The compound , showing structural similarities to both phenytoin and dopamine , was found to decrease spontaneous motor activity of mice and to exert a pronounced protective effect against convulsive seizures induced by pentylenetetrazol ( Metrazol ) .
	manualset3
144643	5	409234	5	NULL	NULL	0	NULL	spontaneous motor activity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The compound , showing structural similarities to both phenytoin and dopamine , was found to decrease spontaneous motor activity of mice and to exert a pronounced protective effect against convulsive seizures induced by pentylenetetrazol ( Metrazol ) .
	manualset3
144644	6	409234	5	NULL	NULL	0	NULL	mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The compound , showing structural similarities to both phenytoin and dopamine , was found to decrease spontaneous motor activity of mice and to exert a pronounced protective effect against convulsive seizures induced by pentylenetetrazol ( Metrazol ) .
	manualset3
144645	7	409234	5	NULL	NULL	0	NULL	protective effect 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The compound , showing structural similarities to both phenytoin and dopamine , was found to decrease spontaneous motor activity of mice and to exert a pronounced protective effect against convulsive seizures induced by pentylenetetrazol ( Metrazol ) .
	manualset3
144646	8	409234	5	NULL	NULL	0	NULL	convulsive seizures 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The compound , showing structural similarities to both phenytoin and dopamine , was found to decrease spontaneous motor activity of mice and to exert a pronounced protective effect against convulsive seizures induced by pentylenetetrazol ( Metrazol ) .
	manualset3
144647	9	409234	5	NULL	NULL	NULL	NULL	pentylenetetrazol ( Metrazol ) 	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The compound , showing structural similarities to both phenytoin and dopamine , was found to decrease spontaneous motor activity of mice and to exert a pronounced protective effect against convulsive seizures induced by pentylenetetrazol ( Metrazol ) .
	manualset3
144648	1	409235	5	NULL	NULL	0	NULL	compound 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The compound exhibited growth inhibitory activity in artificial diet bioassays , with 24.2 and 21.5 ppm , respectively , inhibiting growth by 50 % .
	manualset3
144649	2	409235	5	NULL	NULL	0	NULL	growth inhibitory activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The compound exhibited growth inhibitory activity in artificial diet bioassays , with 24.2 and 21.5 ppm , respectively , inhibiting growth by 50 % .
	manualset3
144650	3	409235	5	NULL	NULL	0	NULL	artificial diet bioassays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The compound exhibited growth inhibitory activity in artificial diet bioassays , with 24.2 and 21.5 ppm , respectively , inhibiting growth by 50 % .
	manualset3
144651	4	409235	5	NULL	NULL	0	NULL	24.2 ppm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The compound exhibited growth inhibitory activity in artificial diet bioassays , with 24.2 and 21.5 ppm , respectively , inhibiting growth by 50 % .
	manualset3
144652	5	409235	5	NULL	NULL	0	NULL	21.5 ppm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The compound exhibited growth inhibitory activity in artificial diet bioassays , with 24.2 and 21.5 ppm , respectively , inhibiting growth by 50 % .
	manualset3
144653	6	409235	5	NULL	NULL	0	NULL	growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The compound exhibited growth inhibitory activity in artificial diet bioassays , with 24.2 and 21.5 ppm , respectively , inhibiting growth by 50 % .
	manualset3
144654	7	409235	5	NULL	NULL	0	NULL	50 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The compound exhibited growth inhibitory activity in artificial diet bioassays , with 24.2 and 21.5 ppm , respectively , inhibiting growth by 50 % .
	manualset3
144655	1	409236	5	NULL	NULL	0	NULL	compound 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The compound is diamagnetic and has only two electrons for metal-metal bonding .
	manualset3
144656	2	409236	5	NULL	NULL	NULL	NULL	two electrons 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The compound is diamagnetic and has only two electrons for metal-metal bonding .
	manualset3
144657	3	409236	5	NULL	NULL	0	NULL	metal-metal bonding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The compound is diamagnetic and has only two electrons for metal-metal bonding .
	manualset3
144658	1	409237	5	NULL	NULL	0	NULL	compounds 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) methyl nitrate ( C1 ) , ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) ethyl nitrate ( C2 ) , 3 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) benzyl nitrate ( C3 ) , 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) - N-hydroxy-benzenesulfonamide ( C4 ) , 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) benzyl nitrate ( C5 ) , and 2 - ( 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) phenyl ) ethyl nitrate ( C6 ) were evaluated with a micronucleus test using mouse peripheral blood to identify new candidate drugs for the treatment of sickle cell disease ( SCD ) that are safer than hydroxyurea .
	manualset3
144659	2	409237	5	NULL	NULL	NULL	NULL	1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) methyl nitrate ( C1 ) 	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The compounds 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) methyl nitrate ( C1 ) , ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) ethyl nitrate ( C2 ) , 3 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) benzyl nitrate ( C3 ) , 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) - N-hydroxy-benzenesulfonamide ( C4 ) , 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) benzyl nitrate ( C5 ) , and 2 - ( 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) phenyl ) ethyl nitrate ( C6 ) were evaluated with a micronucleus test using mouse peripheral blood to identify new candidate drugs for the treatment of sickle cell disease ( SCD ) that are safer than hydroxyurea .
	manualset3
144660	3	409237	5	NULL	NULL	NULL	NULL	( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) ethyl nitrate ( C2 )	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The compounds 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) methyl nitrate ( C1 ) , ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) ethyl nitrate ( C2 ) , 3 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) benzyl nitrate ( C3 ) , 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) - N-hydroxy-benzenesulfonamide ( C4 ) , 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) benzyl nitrate ( C5 ) , and 2 - ( 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) phenyl ) ethyl nitrate ( C6 ) were evaluated with a micronucleus test using mouse peripheral blood to identify new candidate drugs for the treatment of sickle cell disease ( SCD ) that are safer than hydroxyurea .
	manualset3
144661	4	409237	5	NULL	NULL	NULL	NULL	3 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) benzyl nitrate ( C3 )	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The compounds 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) methyl nitrate ( C1 ) , ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) ethyl nitrate ( C2 ) , 3 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) benzyl nitrate ( C3 ) , 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) - N-hydroxy-benzenesulfonamide ( C4 ) , 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) benzyl nitrate ( C5 ) , and 2 - ( 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) phenyl ) ethyl nitrate ( C6 ) were evaluated with a micronucleus test using mouse peripheral blood to identify new candidate drugs for the treatment of sickle cell disease ( SCD ) that are safer than hydroxyurea .
	manualset3
144662	5	409237	5	NULL	NULL	NULL	NULL	4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) - N-hydroxy-benzenesulfonamide ( C4 )	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The compounds 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) methyl nitrate ( C1 ) , ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) ethyl nitrate ( C2 ) , 3 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) benzyl nitrate ( C3 ) , 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) - N-hydroxy-benzenesulfonamide ( C4 ) , 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) benzyl nitrate ( C5 ) , and 2 - ( 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) phenyl ) ethyl nitrate ( C6 ) were evaluated with a micronucleus test using mouse peripheral blood to identify new candidate drugs for the treatment of sickle cell disease ( SCD ) that are safer than hydroxyurea .
	manualset3
144663	6	409237	5	NULL	NULL	0	NULL	4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) benzyl nitrate ( C5 )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) methyl nitrate ( C1 ) , ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) ethyl nitrate ( C2 ) , 3 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) benzyl nitrate ( C3 ) , 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) - N-hydroxy-benzenesulfonamide ( C4 ) , 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) benzyl nitrate ( C5 ) , and 2 - ( 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) phenyl ) ethyl nitrate ( C6 ) were evaluated with a micronucleus test using mouse peripheral blood to identify new candidate drugs for the treatment of sickle cell disease ( SCD ) that are safer than hydroxyurea .
	manualset3
144664	7	409237	5	NULL	NULL	0	NULL	2 - ( 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) phenyl ) ethyl nitrate ( C6 ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) methyl nitrate ( C1 ) , ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) ethyl nitrate ( C2 ) , 3 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) benzyl nitrate ( C3 ) , 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) - N-hydroxy-benzenesulfonamide ( C4 ) , 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) benzyl nitrate ( C5 ) , and 2 - ( 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) phenyl ) ethyl nitrate ( C6 ) were evaluated with a micronucleus test using mouse peripheral blood to identify new candidate drugs for the treatment of sickle cell disease ( SCD ) that are safer than hydroxyurea .
	manualset3
144665	8	409237	5	NULL	NULL	0	NULL	micronucleus test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) methyl nitrate ( C1 ) , ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) ethyl nitrate ( C2 ) , 3 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) benzyl nitrate ( C3 ) , 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) - N-hydroxy-benzenesulfonamide ( C4 ) , 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) benzyl nitrate ( C5 ) , and 2 - ( 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) phenyl ) ethyl nitrate ( C6 ) were evaluated with a micronucleus test using mouse peripheral blood to identify new candidate drugs for the treatment of sickle cell disease ( SCD ) that are safer than hydroxyurea .
	manualset3
144666	9	409237	5	NULL	NULL	0	NULL	mouse peripheral blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) methyl nitrate ( C1 ) , ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) ethyl nitrate ( C2 ) , 3 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) benzyl nitrate ( C3 ) , 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) - N-hydroxy-benzenesulfonamide ( C4 ) , 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) benzyl nitrate ( C5 ) , and 2 - ( 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) phenyl ) ethyl nitrate ( C6 ) were evaluated with a micronucleus test using mouse peripheral blood to identify new candidate drugs for the treatment of sickle cell disease ( SCD ) that are safer than hydroxyurea .
	manualset3
144667	10	409237	5	NULL	NULL	0	NULL	candidate drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) methyl nitrate ( C1 ) , ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) ethyl nitrate ( C2 ) , 3 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) benzyl nitrate ( C3 ) , 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) - N-hydroxy-benzenesulfonamide ( C4 ) , 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) benzyl nitrate ( C5 ) , and 2 - ( 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) phenyl ) ethyl nitrate ( C6 ) were evaluated with a micronucleus test using mouse peripheral blood to identify new candidate drugs for the treatment of sickle cell disease ( SCD ) that are safer than hydroxyurea .
	manualset3
144668	11	409237	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) methyl nitrate ( C1 ) , ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) ethyl nitrate ( C2 ) , 3 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) benzyl nitrate ( C3 ) , 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) - N-hydroxy-benzenesulfonamide ( C4 ) , 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) benzyl nitrate ( C5 ) , and 2 - ( 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) phenyl ) ethyl nitrate ( C6 ) were evaluated with a micronucleus test using mouse peripheral blood to identify new candidate drugs for the treatment of sickle cell disease ( SCD ) that are safer than hydroxyurea .
	manualset3
144669	12	409237	5	NULL	NULL	0	NULL	sickle cell disease ( SCD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) methyl nitrate ( C1 ) , ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) ethyl nitrate ( C2 ) , 3 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) benzyl nitrate ( C3 ) , 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) - N-hydroxy-benzenesulfonamide ( C4 ) , 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) benzyl nitrate ( C5 ) , and 2 - ( 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) phenyl ) ethyl nitrate ( C6 ) were evaluated with a micronucleus test using mouse peripheral blood to identify new candidate drugs for the treatment of sickle cell disease ( SCD ) that are safer than hydroxyurea .
	manualset3
144670	13	409237	5	NULL	NULL	0	NULL	hydroxyurea 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) methyl nitrate ( C1 ) , ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) ethyl nitrate ( C2 ) , 3 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) benzyl nitrate ( C3 ) , 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) - N-hydroxy-benzenesulfonamide ( C4 ) , 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) benzyl nitrate ( C5 ) , and 2 - ( 4 - ( 1 , 3-dioxo-1 , 3 - dihydro-2H-isoindol-2-yl ) phenyl ) ethyl nitrate ( C6 ) were evaluated with a micronucleus test using mouse peripheral blood to identify new candidate drugs for the treatment of sickle cell disease ( SCD ) that are safer than hydroxyurea .
	manualset3
144671	1	409238	5	NULL	NULL	0	NULL	compounds 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds Ru ( bpy ) 2 ( BTL ) ( PF 6 ) 2 and Ru ( deeb ) 2 ( BTL ) ( PF 6 ) 2 , where bpy is 2 , 2 ' - bipyridine , deeb is 4 , 4 ' - ( C 2H 5CO 2 ) 2-bpy , and BTL is 9 ' - ( 4 , 5-bis ( cyanoethylthio ) ) -1 , 3 - dithiol-2-ylidene ) -4 ' , 5 ' - diazafluorene , were found to have very high extinction coefficients in the visible region .
	manualset3
144672	2	409238	5	NULL	NULL	0	NULL	compounds 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds Ru ( bpy ) 2 ( BTL ) ( PF 6 ) 2 and Ru ( deeb ) 2 ( BTL ) ( PF 6 ) 2 , where bpy is 2 , 2 ' - bipyridine , deeb is 4 , 4 ' - ( C 2H 5CO 2 ) 2-bpy , and BTL is 9 ' - ( 4 , 5-bis ( cyanoethylthio ) ) -1 , 3 - dithiol-2-ylidene ) -4 ' , 5 ' - diazafluorene , were found to have very high extinction coefficients in the visible region .
	manualset3
144673	3	409238	5	NULL	NULL	0	NULL	Ru ( bpy ) 2 ( BTL ) ( PF 6 ) 2 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds Ru ( bpy ) 2 ( BTL ) ( PF 6 ) 2 and Ru ( deeb ) 2 ( BTL ) ( PF 6 ) 2 , where bpy is 2 , 2 ' - bipyridine , deeb is 4 , 4 ' - ( C 2H 5CO 2 ) 2-bpy , and BTL is 9 ' - ( 4 , 5-bis ( cyanoethylthio ) ) -1 , 3 - dithiol-2-ylidene ) -4 ' , 5 ' - diazafluorene , were found to have very high extinction coefficients in the visible region .
	manualset3
144674	4	409238	5	NULL	NULL	0	NULL	Ru ( deeb ) 2 ( BTL ) ( PF 6 ) 2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds Ru ( bpy ) 2 ( BTL ) ( PF 6 ) 2 and Ru ( deeb ) 2 ( BTL ) ( PF 6 ) 2 , where bpy is 2 , 2 ' - bipyridine , deeb is 4 , 4 ' - ( C 2H 5CO 2 ) 2-bpy , and BTL is 9 ' - ( 4 , 5-bis ( cyanoethylthio ) ) -1 , 3 - dithiol-2-ylidene ) -4 ' , 5 ' - diazafluorene , were found to have very high extinction coefficients in the visible region .
	manualset3
144675	5	409238	5	NULL	NULL	NULL	NULL	bpy 	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The compounds Ru ( bpy ) 2 ( BTL ) ( PF 6 ) 2 and Ru ( deeb ) 2 ( BTL ) ( PF 6 ) 2 , where bpy is 2 , 2 ' - bipyridine , deeb is 4 , 4 ' - ( C 2H 5CO 2 ) 2-bpy , and BTL is 9 ' - ( 4 , 5-bis ( cyanoethylthio ) ) -1 , 3 - dithiol-2-ylidene ) -4 ' , 5 ' - diazafluorene , were found to have very high extinction coefficients in the visible region .
	manualset3
144676	6	409238	5	NULL	NULL	0	NULL	2 , 2 ' - bipyridine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds Ru ( bpy ) 2 ( BTL ) ( PF 6 ) 2 and Ru ( deeb ) 2 ( BTL ) ( PF 6 ) 2 , where bpy is 2 , 2 ' - bipyridine , deeb is 4 , 4 ' - ( C 2H 5CO 2 ) 2-bpy , and BTL is 9 ' - ( 4 , 5-bis ( cyanoethylthio ) ) -1 , 3 - dithiol-2-ylidene ) -4 ' , 5 ' - diazafluorene , were found to have very high extinction coefficients in the visible region .
	manualset3
144677	7	409238	5	NULL	NULL	0	NULL	deeb 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds Ru ( bpy ) 2 ( BTL ) ( PF 6 ) 2 and Ru ( deeb ) 2 ( BTL ) ( PF 6 ) 2 , where bpy is 2 , 2 ' - bipyridine , deeb is 4 , 4 ' - ( C 2H 5CO 2 ) 2-bpy , and BTL is 9 ' - ( 4 , 5-bis ( cyanoethylthio ) ) -1 , 3 - dithiol-2-ylidene ) -4 ' , 5 ' - diazafluorene , were found to have very high extinction coefficients in the visible region .
	manualset3
144678	8	409238	5	NULL	NULL	0	NULL	4 , 4 ' - ( C 2H 5CO 2 ) 2-bpy	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds Ru ( bpy ) 2 ( BTL ) ( PF 6 ) 2 and Ru ( deeb ) 2 ( BTL ) ( PF 6 ) 2 , where bpy is 2 , 2 ' - bipyridine , deeb is 4 , 4 ' - ( C 2H 5CO 2 ) 2-bpy , and BTL is 9 ' - ( 4 , 5-bis ( cyanoethylthio ) ) -1 , 3 - dithiol-2-ylidene ) -4 ' , 5 ' - diazafluorene , were found to have very high extinction coefficients in the visible region .
	manualset3
144679	9	409238	5	NULL	NULL	0	NULL	BTL 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds Ru ( bpy ) 2 ( BTL ) ( PF 6 ) 2 and Ru ( deeb ) 2 ( BTL ) ( PF 6 ) 2 , where bpy is 2 , 2 ' - bipyridine , deeb is 4 , 4 ' - ( C 2H 5CO 2 ) 2-bpy , and BTL is 9 ' - ( 4 , 5-bis ( cyanoethylthio ) ) -1 , 3 - dithiol-2-ylidene ) -4 ' , 5 ' - diazafluorene , were found to have very high extinction coefficients in the visible region .
	manualset3
144680	10	409238	5	NULL	NULL	0	NULL	9 ' - ( 4 , 5-bis ( cyanoethylthio ) ) -1 , 3 - dithiol-2-ylidene ) -4 ' , 5 ' - diazafluorene 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds Ru ( bpy ) 2 ( BTL ) ( PF 6 ) 2 and Ru ( deeb ) 2 ( BTL ) ( PF 6 ) 2 , where bpy is 2 , 2 ' - bipyridine , deeb is 4 , 4 ' - ( C 2H 5CO 2 ) 2-bpy , and BTL is 9 ' - ( 4 , 5-bis ( cyanoethylthio ) ) -1 , 3 - dithiol-2-ylidene ) -4 ' , 5 ' - diazafluorene , were found to have very high extinction coefficients in the visible region .
	manualset3
144681	11	409238	5	NULL	NULL	0	NULL	extinction coefficients	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds Ru ( bpy ) 2 ( BTL ) ( PF 6 ) 2 and Ru ( deeb ) 2 ( BTL ) ( PF 6 ) 2 , where bpy is 2 , 2 ' - bipyridine , deeb is 4 , 4 ' - ( C 2H 5CO 2 ) 2-bpy , and BTL is 9 ' - ( 4 , 5-bis ( cyanoethylthio ) ) -1 , 3 - dithiol-2-ylidene ) -4 ' , 5 ' - diazafluorene , were found to have very high extinction coefficients in the visible region .
	manualset3
144682	12	409238	5	NULL	NULL	0	NULL	visible region	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds Ru ( bpy ) 2 ( BTL ) ( PF 6 ) 2 and Ru ( deeb ) 2 ( BTL ) ( PF 6 ) 2 , where bpy is 2 , 2 ' - bipyridine , deeb is 4 , 4 ' - ( C 2H 5CO 2 ) 2-bpy , and BTL is 9 ' - ( 4 , 5-bis ( cyanoethylthio ) ) -1 , 3 - dithiol-2-ylidene ) -4 ' , 5 ' - diazafluorene , were found to have very high extinction coefficients in the visible region .
	manualset3
144683	1	409239	5	NULL	NULL	0	NULL	elevation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant elevation of VIII C over VIII C : Ag values was observed in children with poor actual control of diabetes , but no elevation of VIII C over VIII C : Ag was found in children with good actual control .
	manualset3
144684	2	409239	5	NULL	NULL	0	NULL	VIII C 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant elevation of VIII C over VIII C : Ag values was observed in children with poor actual control of diabetes , but no elevation of VIII C over VIII C : Ag was found in children with good actual control .
	manualset3
144685	3	409239	5	NULL	NULL	0	NULL	VIII C : Ag values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant elevation of VIII C over VIII C : Ag values was observed in children with poor actual control of diabetes , but no elevation of VIII C over VIII C : Ag was found in children with good actual control .
	manualset3
144686	4	409239	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant elevation of VIII C over VIII C : Ag values was observed in children with poor actual control of diabetes , but no elevation of VIII C over VIII C : Ag was found in children with good actual control .
	manualset3
144688	5	409239	5	NULL	NULL	0	NULL	diabetes 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant elevation of VIII C over VIII C : Ag values was observed in children with poor actual control of diabetes , but no elevation of VIII C over VIII C : Ag was found in children with good actual control .
	manualset3
144689	6	409239	5	NULL	NULL	0	NULL	elevation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant elevation of VIII C over VIII C : Ag values was observed in children with poor actual control of diabetes , but no elevation of VIII C over VIII C : Ag was found in children with good actual control .
	manualset3
144690	7	409239	5	NULL	NULL	0	NULL	VIII C	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant elevation of VIII C over VIII C : Ag values was observed in children with poor actual control of diabetes , but no elevation of VIII C over VIII C : Ag was found in children with good actual control .
	manualset3
144691	8	409239	5	NULL	NULL	0	NULL	VIII C : Ag	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant elevation of VIII C over VIII C : Ag values was observed in children with poor actual control of diabetes , but no elevation of VIII C over VIII C : Ag was found in children with good actual control .
	manualset3
144692	9	409239	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant elevation of VIII C over VIII C : Ag values was observed in children with poor actual control of diabetes , but no elevation of VIII C over VIII C : Ag was found in children with good actual control .
	manualset3
144693	1	409240	5	NULL	NULL	0	NULL	compounds 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds belong to the following groups : BTEX , C3-benzenes , bicyclo compounds , napthalenes , chlorinated aliphatics , phenols ( chloro - , methyl - , dimethyl , nonyl - ) , pesticides , and phthalates .
	manualset3
144694	2	409240	5	NULL	NULL	0	NULL	groups 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds belong to the following groups : BTEX , C3-benzenes , bicyclo compounds , napthalenes , chlorinated aliphatics , phenols ( chloro - , methyl - , dimethyl , nonyl - ) , pesticides , and phthalates .
	manualset3
144695	3	409240	5	NULL	NULL	0	NULL	BTEX 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds belong to the following groups : BTEX , C3-benzenes , bicyclo compounds , napthalenes , chlorinated aliphatics , phenols ( chloro - , methyl - , dimethyl , nonyl - ) , pesticides , and phthalates .
	manualset3
144696	4	409240	5	NULL	NULL	0	NULL	C3-benzenes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds belong to the following groups : BTEX , C3-benzenes , bicyclo compounds , napthalenes , chlorinated aliphatics , phenols ( chloro - , methyl - , dimethyl , nonyl - ) , pesticides , and phthalates .
	manualset3
144697	5	409240	5	NULL	NULL	0	NULL	bicyclo compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds belong to the following groups : BTEX , C3-benzenes , bicyclo compounds , napthalenes , chlorinated aliphatics , phenols ( chloro - , methyl - , dimethyl , nonyl - ) , pesticides , and phthalates .
	manualset3
144698	6	409240	5	NULL	NULL	0	NULL	napthalenes 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds belong to the following groups : BTEX , C3-benzenes , bicyclo compounds , napthalenes , chlorinated aliphatics , phenols ( chloro - , methyl - , dimethyl , nonyl - ) , pesticides , and phthalates .
	manualset3
144699	7	409240	5	NULL	NULL	0	NULL	chlorinated aliphatics	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds belong to the following groups : BTEX , C3-benzenes , bicyclo compounds , napthalenes , chlorinated aliphatics , phenols ( chloro - , methyl - , dimethyl , nonyl - ) , pesticides , and phthalates .
	manualset3
144700	8	409240	5	NULL	NULL	0	NULL	phenols ( chloro - , methyl - , dimethyl , nonyl - ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds belong to the following groups : BTEX , C3-benzenes , bicyclo compounds , napthalenes , chlorinated aliphatics , phenols ( chloro - , methyl - , dimethyl , nonyl - ) , pesticides , and phthalates .
	manualset3
144701	9	409240	5	NULL	NULL	0	NULL	pesticides 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds belong to the following groups : BTEX , C3-benzenes , bicyclo compounds , napthalenes , chlorinated aliphatics , phenols ( chloro - , methyl - , dimethyl , nonyl - ) , pesticides , and phthalates .
	manualset3
144702	10	409240	5	NULL	NULL	0	NULL	phthalates 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds belong to the following groups : BTEX , C3-benzenes , bicyclo compounds , napthalenes , chlorinated aliphatics , phenols ( chloro - , methyl - , dimethyl , nonyl - ) , pesticides , and phthalates .
	manualset3
144703	1	409241	5	NULL	NULL	0	NULL	compounds 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds under study were divided arbitrarily into two groups : water soluble ( ) 10 g/l ) and slightly soluble in water ( & lt ; 10 g/l ) compounds .
	manualset3
144704	2	409241	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds under study were divided arbitrarily into two groups : water soluble ( ) 10 g/l ) and slightly soluble in water ( & lt ; 10 g/l ) compounds .
	manualset3
144705	3	409241	5	NULL	NULL	0	NULL	two groups 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds under study were divided arbitrarily into two groups : water soluble ( ) 10 g/l ) and slightly soluble in water ( & lt ; 10 g/l ) compounds .
	manualset3
144706	4	409241	5	NULL	NULL	NULL	NULL	water soluble compounds	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The compounds under study were divided arbitrarily into two groups : water soluble ( ) 10 g/l ) and slightly soluble in water ( & lt ; 10 g/l ) compounds .
	manualset3
144707	5	409241	5	NULL	NULL	0	NULL	10 g/l 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds under study were divided arbitrarily into two groups : water soluble ( ) 10 g/l ) and slightly soluble in water ( & lt ; 10 g/l ) compounds .
	manualset3
144708	6	409241	5	NULL	NULL	NULL	NULL	slightly soluble in water compounds	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The compounds under study were divided arbitrarily into two groups : water soluble ( ) 10 g/l ) and slightly soluble in water ( & lt ; 10 g/l ) compounds .
	manualset3
144709	7	409241	5	NULL	NULL	0	NULL	& lt ; 10 g/l	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds under study were divided arbitrarily into two groups : water soluble ( ) 10 g/l ) and slightly soluble in water ( & lt ; 10 g/l ) compounds .
	manualset3
144710	1	409242	5	NULL	NULL	0	NULL	compounds 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds were identified as 5 , 7 , 5 ' - trihydroxy-3 , 6 , 2 ' , 4 ' - tetramethoxyflavone ( 1 ) , scopoletin ( 2 ) and centaureidin ( 3 ) which inhibited the edema by 67.3 % , 59.8 % and 49.7 % , respectively , at a dose of 1 mg/ear .
	manualset3
144711	2	409242	5	NULL	NULL	0	NULL	5 , 7 , 5 ' - trihydroxy-3 , 6 , 2 ' , 4 ' - tetramethoxyflavone ( 1 ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds were identified as 5 , 7 , 5 ' - trihydroxy-3 , 6 , 2 ' , 4 ' - tetramethoxyflavone ( 1 ) , scopoletin ( 2 ) and centaureidin ( 3 ) which inhibited the edema by 67.3 % , 59.8 % and 49.7 % , respectively , at a dose of 1 mg/ear .
	manualset3
144712	3	409242	5	NULL	NULL	0	NULL	scopoletin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds were identified as 5 , 7 , 5 ' - trihydroxy-3 , 6 , 2 ' , 4 ' - tetramethoxyflavone ( 1 ) , scopoletin ( 2 ) and centaureidin ( 3 ) which inhibited the edema by 67.3 % , 59.8 % and 49.7 % , respectively , at a dose of 1 mg/ear .
	manualset3
144713	4	409242	5	NULL	NULL	0	NULL	centaureidin 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds were identified as 5 , 7 , 5 ' - trihydroxy-3 , 6 , 2 ' , 4 ' - tetramethoxyflavone ( 1 ) , scopoletin ( 2 ) and centaureidin ( 3 ) which inhibited the edema by 67.3 % , 59.8 % and 49.7 % , respectively , at a dose of 1 mg/ear .
	manualset3
144714	5	409242	5	NULL	NULL	0	NULL	edema 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds were identified as 5 , 7 , 5 ' - trihydroxy-3 , 6 , 2 ' , 4 ' - tetramethoxyflavone ( 1 ) , scopoletin ( 2 ) and centaureidin ( 3 ) which inhibited the edema by 67.3 % , 59.8 % and 49.7 % , respectively , at a dose of 1 mg/ear .
	manualset3
144715	6	409242	5	NULL	NULL	0	NULL	67.3 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds were identified as 5 , 7 , 5 ' - trihydroxy-3 , 6 , 2 ' , 4 ' - tetramethoxyflavone ( 1 ) , scopoletin ( 2 ) and centaureidin ( 3 ) which inhibited the edema by 67.3 % , 59.8 % and 49.7 % , respectively , at a dose of 1 mg/ear .
	manualset3
144716	7	409242	5	NULL	NULL	0	NULL	59.8 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds were identified as 5 , 7 , 5 ' - trihydroxy-3 , 6 , 2 ' , 4 ' - tetramethoxyflavone ( 1 ) , scopoletin ( 2 ) and centaureidin ( 3 ) which inhibited the edema by 67.3 % , 59.8 % and 49.7 % , respectively , at a dose of 1 mg/ear .
	manualset3
144717	8	409242	5	NULL	NULL	0	NULL	 49.7 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds were identified as 5 , 7 , 5 ' - trihydroxy-3 , 6 , 2 ' , 4 ' - tetramethoxyflavone ( 1 ) , scopoletin ( 2 ) and centaureidin ( 3 ) which inhibited the edema by 67.3 % , 59.8 % and 49.7 % , respectively , at a dose of 1 mg/ear .
	manualset3
144718	9	409242	5	NULL	NULL	0	NULL	dose 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds were identified as 5 , 7 , 5 ' - trihydroxy-3 , 6 , 2 ' , 4 ' - tetramethoxyflavone ( 1 ) , scopoletin ( 2 ) and centaureidin ( 3 ) which inhibited the edema by 67.3 % , 59.8 % and 49.7 % , respectively , at a dose of 1 mg/ear .
	manualset3
144719	10	409242	5	NULL	NULL	0	NULL	1 mg/ear	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds were identified as 5 , 7 , 5 ' - trihydroxy-3 , 6 , 2 ' , 4 ' - tetramethoxyflavone ( 1 ) , scopoletin ( 2 ) and centaureidin ( 3 ) which inhibited the edema by 67.3 % , 59.8 % and 49.7 % , respectively , at a dose of 1 mg/ear .
	manualset3
144720	1	409243	5	NULL	NULL	0	NULL	compounds 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds were tested in a DPPH assay , in antimicrobial assays against bacteria , yeasts , and fungi , and in antiproliferation assays using cultures of mouse fibroblasts .
	manualset3
144721	2	409243	5	NULL	NULL	0	NULL	DPPH assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds were tested in a DPPH assay , in antimicrobial assays against bacteria , yeasts , and fungi , and in antiproliferation assays using cultures of mouse fibroblasts .
	manualset3
144722	3	409243	5	NULL	NULL	0	NULL	antimicrobial assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds were tested in a DPPH assay , in antimicrobial assays against bacteria , yeasts , and fungi , and in antiproliferation assays using cultures of mouse fibroblasts .
	manualset3
144723	4	409243	5	NULL	NULL	0	NULL	bacteria 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds were tested in a DPPH assay , in antimicrobial assays against bacteria , yeasts , and fungi , and in antiproliferation assays using cultures of mouse fibroblasts .
	manualset3
144724	5	409243	5	NULL	NULL	0	NULL	yeasts 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds were tested in a DPPH assay , in antimicrobial assays against bacteria , yeasts , and fungi , and in antiproliferation assays using cultures of mouse fibroblasts .
	manualset3
144725	6	409243	5	NULL	NULL	0	NULL	fungi 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds were tested in a DPPH assay , in antimicrobial assays against bacteria , yeasts , and fungi , and in antiproliferation assays using cultures of mouse fibroblasts .
	manualset3
144726	7	409243	5	NULL	NULL	0	NULL	antiproliferation assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The compounds were tested in a DPPH assay , in antimicrobial assays against bacteria , yeasts , and fungi , and in antiproliferation assays using cultures of mouse fibroblasts .
	manualset3
144727	8	409243	5	NULL	NULL	NULL	NULL	cultures of mouse fibroblasts	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The compounds were tested in a DPPH assay , in antimicrobial assays against bacteria , yeasts , and fungi , and in antiproliferation assays using cultures of mouse fibroblasts .
	manualset3
144728	1	409244	5	NULL	NULL	0	NULL	computations 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The computations imply that the new radical cation S ( 4 ) ( + ) may be present in sulfur dioxide solutions given on reaction of sulfur oxidized by AsF ( 5 ) in the presence of a facilitating agent .
	manualset3
144729	2	409244	5	NULL	NULL	0	NULL	new radical cation S ( 4 ) ( + ) 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The computations imply that the new radical cation S ( 4 ) ( + ) may be present in sulfur dioxide solutions given on reaction of sulfur oxidized by AsF ( 5 ) in the presence of a facilitating agent .
	manualset3
144730	3	409244	5	NULL	NULL	0	NULL	sulfur dioxide solutions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The computations imply that the new radical cation S ( 4 ) ( + ) may be present in sulfur dioxide solutions given on reaction of sulfur oxidized by AsF ( 5 ) in the presence of a facilitating agent .
	manualset3
144731	4	409244	5	NULL	NULL	0	NULL	reaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The computations imply that the new radical cation S ( 4 ) ( + ) may be present in sulfur dioxide solutions given on reaction of sulfur oxidized by AsF ( 5 ) in the presence of a facilitating agent .
	manualset3
144732	5	409244	5	NULL	NULL	0	NULL	sulfur 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The computations imply that the new radical cation S ( 4 ) ( + ) may be present in sulfur dioxide solutions given on reaction of sulfur oxidized by AsF ( 5 ) in the presence of a facilitating agent .
	manualset3
144733	6	409244	5	NULL	NULL	0	NULL	AsF ( 5 )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The computations imply that the new radical cation S ( 4 ) ( + ) may be present in sulfur dioxide solutions given on reaction of sulfur oxidized by AsF ( 5 ) in the presence of a facilitating agent .
	manualset3
144734	7	409244	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The computations imply that the new radical cation S ( 4 ) ( + ) may be present in sulfur dioxide solutions given on reaction of sulfur oxidized by AsF ( 5 ) in the presence of a facilitating agent .
	manualset3
144735	8	409244	5	NULL	NULL	0	NULL	facilitating agent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The computations imply that the new radical cation S ( 4 ) ( + ) may be present in sulfur dioxide solutions given on reaction of sulfur oxidized by AsF ( 5 ) in the presence of a facilitating agent .
	manualset3
144736	1	409245	5	NULL	NULL	0	NULL	computed barrier heights	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The computed barrier heights and geometrical parameters of the transition structures are in agreement with Hammond 's postulate , and the relative energies of all of the equilibrium structures can be rationalized by Hckel molecular orbital ( HMO ) theory .
	manualset3
144737	2	409245	5	NULL	NULL	0	NULL	geometrical parameters 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The computed barrier heights and geometrical parameters of the transition structures are in agreement with Hammond 's postulate , and the relative energies of all of the equilibrium structures can be rationalized by Hckel molecular orbital ( HMO ) theory .
	manualset3
144738	3	409245	5	NULL	NULL	0	NULL	transition structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The computed barrier heights and geometrical parameters of the transition structures are in agreement with Hammond 's postulate , and the relative energies of all of the equilibrium structures can be rationalized by Hckel molecular orbital ( HMO ) theory .
	manualset3
144739	4	409245	5	NULL	NULL	0	NULL	agreement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The computed barrier heights and geometrical parameters of the transition structures are in agreement with Hammond 's postulate , and the relative energies of all of the equilibrium structures can be rationalized by Hckel molecular orbital ( HMO ) theory .
	manualset3
144740	5	409245	5	NULL	NULL	0	NULL	Hammond 's postulate	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The computed barrier heights and geometrical parameters of the transition structures are in agreement with Hammond 's postulate , and the relative energies of all of the equilibrium structures can be rationalized by Hckel molecular orbital ( HMO ) theory .
	manualset3
144741	6	409245	5	NULL	NULL	0	NULL	relative energies	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The computed barrier heights and geometrical parameters of the transition structures are in agreement with Hammond 's postulate , and the relative energies of all of the equilibrium structures can be rationalized by Hckel molecular orbital ( HMO ) theory .
	manualset3
144742	7	409245	5	NULL	NULL	0	NULL	equilibrium structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The computed barrier heights and geometrical parameters of the transition structures are in agreement with Hammond 's postulate , and the relative energies of all of the equilibrium structures can be rationalized by Hckel molecular orbital ( HMO ) theory .
	manualset3
144743	8	409245	5	NULL	NULL	0	NULL	Hckel molecular orbital ( HMO ) theory 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The computed barrier heights and geometrical parameters of the transition structures are in agreement with Hammond 's postulate , and the relative energies of all of the equilibrium structures can be rationalized by Hckel molecular orbital ( HMO ) theory .
	manualset3
144744	1	409246	5	NULL	NULL	0	NULL	computer analyses 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The computer analyses predicted that numerous nonapeptides with motifs to bind HLA class I A68 and A2 haplotypes were detected .
	manualset3
144745	2	409246	5	NULL	NULL	0	NULL	numerous nonapeptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The computer analyses predicted that numerous nonapeptides with motifs to bind HLA class I A68 and A2 haplotypes were detected .
	manualset3
144746	3	409246	5	NULL	NULL	0	NULL	motifs 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The computer analyses predicted that numerous nonapeptides with motifs to bind HLA class I A68 and A2 haplotypes were detected .
	manualset3
144747	4	409246	5	NULL	NULL	NULL	NULL	HLA class I A68 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The computer analyses predicted that numerous nonapeptides with motifs to bind HLA class I A68 and A2 haplotypes were detected .
	manualset3
144748	5	409246	5	NULL	NULL	0	NULL	A2 haplotypes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The computer analyses predicted that numerous nonapeptides with motifs to bind HLA class I A68 and A2 haplotypes were detected .
	manualset3
144749	1	409247	5	NULL	NULL	0	NULL	concave mirror	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The concave mirror is fabricated by attaching a thin polycarbonate ( PC ) film on the fiber end , pressing the PC film with a fiber ball to form a dimple , and then depositing a multilayer dielectric mirror .
	manualset3
144750	2	409247	5	NULL	NULL	0	NULL	thin polycarbonate ( PC ) film	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The concave mirror is fabricated by attaching a thin polycarbonate ( PC ) film on the fiber end , pressing the PC film with a fiber ball to form a dimple , and then depositing a multilayer dielectric mirror .
	manualset3
144751	3	409247	5	NULL	NULL	0	NULL	fiber end	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The concave mirror is fabricated by attaching a thin polycarbonate ( PC ) film on the fiber end , pressing the PC film with a fiber ball to form a dimple , and then depositing a multilayer dielectric mirror .
	manualset3
144752	4	409247	5	NULL	NULL	0	NULL	PC film	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The concave mirror is fabricated by attaching a thin polycarbonate ( PC ) film on the fiber end , pressing the PC film with a fiber ball to form a dimple , and then depositing a multilayer dielectric mirror .
	manualset3
144753	5	409247	5	NULL	NULL	0	NULL	fiber ball	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The concave mirror is fabricated by attaching a thin polycarbonate ( PC ) film on the fiber end , pressing the PC film with a fiber ball to form a dimple , and then depositing a multilayer dielectric mirror .
	manualset3
144754	6	409247	5	NULL	NULL	0	NULL	dimple 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concave mirror is fabricated by attaching a thin polycarbonate ( PC ) film on the fiber end , pressing the PC film with a fiber ball to form a dimple , and then depositing a multilayer dielectric mirror .
	manualset3
144755	7	409247	5	NULL	NULL	0	NULL	multilayer dielectric mirror	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The concave mirror is fabricated by attaching a thin polycarbonate ( PC ) film on the fiber end , pressing the PC film with a fiber ball to form a dimple , and then depositing a multilayer dielectric mirror .
	manualset3
144756	1	409248	5	NULL	NULL	0	NULL	concentration-relaxation curve	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration-relaxation curve of 2-chloroadenosine was not altered by reactive red 2 .
	manualset3
144757	2	409248	5	NULL	NULL	0	NULL	2-chloroadenosine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration-relaxation curve of 2-chloroadenosine was not altered by reactive red 2 .
	manualset3
144758	3	409248	5	NULL	NULL	0	NULL	reactive red 2	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration-relaxation curve of 2-chloroadenosine was not altered by reactive red 2 .
	manualset3
144759	1	409249	5	NULL	NULL	0	NULL	Chronic endophthalmitis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Chronic endophthalmitis due to Toxocara canis ) .
	manualset3
144760	2	409249	5	NULL	NULL	0	NULL	Toxocara canis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Chronic endophthalmitis due to Toxocara canis ) .
	manualset3
144761	1	409250	5	NULL	NULL	0	NULL	concentration-response curves 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration-response curves of unlabelled serotonin and noradrenaline for their inhibitory effects on impulse-evoked 3H overflow were shifted to the right by quipazine .
	manualset3
144762	2	409250	5	NULL	NULL	0	NULL	unlabelled serotonin	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration-response curves of unlabelled serotonin and noradrenaline for their inhibitory effects on impulse-evoked 3H overflow were shifted to the right by quipazine .
	manualset3
144763	3	409250	5	NULL	NULL	0	NULL	noradrenaline 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration-response curves of unlabelled serotonin and noradrenaline for their inhibitory effects on impulse-evoked 3H overflow were shifted to the right by quipazine .
	manualset3
144764	4	409250	5	NULL	NULL	0	NULL	inhibitory effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration-response curves of unlabelled serotonin and noradrenaline for their inhibitory effects on impulse-evoked 3H overflow were shifted to the right by quipazine .
	manualset3
144765	5	409250	5	NULL	NULL	0	NULL	impulse-evoked 3H overflow	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration-response curves of unlabelled serotonin and noradrenaline for their inhibitory effects on impulse-evoked 3H overflow were shifted to the right by quipazine .
	manualset3
144766	6	409250	5	NULL	NULL	0	NULL	quipazine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration-response curves of unlabelled serotonin and noradrenaline for their inhibitory effects on impulse-evoked 3H overflow were shifted to the right by quipazine .
	manualset3
144767	1	409251	5	NULL	NULL	0	NULL	concentration - dependent effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration - and time-dependent effects of sulphur mustard on cultured human epidermal keratinocyte function were investigated with respect to cell proliferation , DNA and protein synthesis , the level of NAD ( + ) and ATP , and the intracellular activity of lactate dehydrogenase .
	manualset3
144768	2	409251	5	NULL	NULL	0	NULL	time-dependent effects 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration - and time-dependent effects of sulphur mustard on cultured human epidermal keratinocyte function were investigated with respect to cell proliferation , DNA and protein synthesis , the level of NAD ( + ) and ATP , and the intracellular activity of lactate dehydrogenase .
	manualset3
144769	3	409251	5	NULL	NULL	0	NULL	sulphur mustard	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration - and time-dependent effects of sulphur mustard on cultured human epidermal keratinocyte function were investigated with respect to cell proliferation , DNA and protein synthesis , the level of NAD ( + ) and ATP , and the intracellular activity of lactate dehydrogenase .
	manualset3
144770	4	409251	5	NULL	NULL	0	NULL	cultured human epidermal keratinocyte function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration - and time-dependent effects of sulphur mustard on cultured human epidermal keratinocyte function were investigated with respect to cell proliferation , DNA and protein synthesis , the level of NAD ( + ) and ATP , and the intracellular activity of lactate dehydrogenase .
	manualset3
144771	5	409251	5	NULL	NULL	0	NULL	cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration - and time-dependent effects of sulphur mustard on cultured human epidermal keratinocyte function were investigated with respect to cell proliferation , DNA and protein synthesis , the level of NAD ( + ) and ATP , and the intracellular activity of lactate dehydrogenase .
	manualset3
144772	6	409251	5	NULL	NULL	0	NULL	DNA synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration - and time-dependent effects of sulphur mustard on cultured human epidermal keratinocyte function were investigated with respect to cell proliferation , DNA and protein synthesis , the level of NAD ( + ) and ATP , and the intracellular activity of lactate dehydrogenase .
	manualset3
144773	7	409251	5	NULL	NULL	0	NULL	protein synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration - and time-dependent effects of sulphur mustard on cultured human epidermal keratinocyte function were investigated with respect to cell proliferation , DNA and protein synthesis , the level of NAD ( + ) and ATP , and the intracellular activity of lactate dehydrogenase .
	manualset3
144774	8	409251	5	NULL	NULL	0	NULL	level of NAD ( + ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration - and time-dependent effects of sulphur mustard on cultured human epidermal keratinocyte function were investigated with respect to cell proliferation , DNA and protein synthesis , the level of NAD ( + ) and ATP , and the intracellular activity of lactate dehydrogenase .
	manualset3
144775	9	409251	5	NULL	NULL	0	NULL	level of ATP	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration - and time-dependent effects of sulphur mustard on cultured human epidermal keratinocyte function were investigated with respect to cell proliferation , DNA and protein synthesis , the level of NAD ( + ) and ATP , and the intracellular activity of lactate dehydrogenase .
	manualset3
144776	10	409251	5	NULL	NULL	0	NULL	intracellular activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration - and time-dependent effects of sulphur mustard on cultured human epidermal keratinocyte function were investigated with respect to cell proliferation , DNA and protein synthesis , the level of NAD ( + ) and ATP , and the intracellular activity of lactate dehydrogenase .
	manualset3
144777	11	409251	5	NULL	NULL	0	NULL	lactate dehydrogenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration - and time-dependent effects of sulphur mustard on cultured human epidermal keratinocyte function were investigated with respect to cell proliferation , DNA and protein synthesis , the level of NAD ( + ) and ATP , and the intracellular activity of lactate dehydrogenase .
	manualset3
144778	1	409252	5	NULL	NULL	0	NULL	concentration -dependence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration - and voltage-dependence of the steady-state block of the inward rectifying K + current ( IK1 ) was fitted by a simple model assuming 1 : 1 binding of Ba2 + to a site within the membrane .
	manualset3
144779	2	409252	5	NULL	NULL	0	NULL	voltage-dependence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration - and voltage-dependence of the steady-state block of the inward rectifying K + current ( IK1 ) was fitted by a simple model assuming 1 : 1 binding of Ba2 + to a site within the membrane .
	manualset3
144780	3	409252	5	NULL	NULL	0	NULL	steady-state block	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration - and voltage-dependence of the steady-state block of the inward rectifying K + current ( IK1 ) was fitted by a simple model assuming 1 : 1 binding of Ba2 + to a site within the membrane .
	manualset3
144781	4	409252	5	NULL	NULL	0	NULL	inward rectifying K + current ( IK1 )	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration - and voltage-dependence of the steady-state block of the inward rectifying K + current ( IK1 ) was fitted by a simple model assuming 1 : 1 binding of Ba2 + to a site within the membrane .
	manualset3
144782	5	409252	5	NULL	NULL	0	NULL	simple model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration - and voltage-dependence of the steady-state block of the inward rectifying K + current ( IK1 ) was fitted by a simple model assuming 1 : 1 binding of Ba2 + to a site within the membrane .
	manualset3
144783	6	409252	5	NULL	NULL	0	NULL	1 : 1 binding	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration - and voltage-dependence of the steady-state block of the inward rectifying K + current ( IK1 ) was fitted by a simple model assuming 1 : 1 binding of Ba2 + to a site within the membrane .
	manualset3
144784	7	409252	5	NULL	NULL	0	NULL	Ba2 + 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration - and voltage-dependence of the steady-state block of the inward rectifying K + current ( IK1 ) was fitted by a simple model assuming 1 : 1 binding of Ba2 + to a site within the membrane .
	manualset3
144785	8	409252	5	NULL	NULL	0	NULL	membrane 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration - and voltage-dependence of the steady-state block of the inward rectifying K + current ( IK1 ) was fitted by a simple model assuming 1 : 1 binding of Ba2 + to a site within the membrane .
	manualset3
144786	1	409253	5	NULL	NULL	NULL	NULL	concentration dependence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The concentration dependence gives evidence that the Coulomb interaction energy is the energy scale that determines this crossover .
	manualset3
144787	2	409253	5	NULL	NULL	0	NULL	evidence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration dependence gives evidence that the Coulomb interaction energy is the energy scale that determines this crossover .
	manualset3
144788	3	409253	5	NULL	NULL	0	NULL	Coulomb interaction energy	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration dependence gives evidence that the Coulomb interaction energy is the energy scale that determines this crossover .
	manualset3
144789	4	409253	5	NULL	NULL	0	NULL	energy scale 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration dependence gives evidence that the Coulomb interaction energy is the energy scale that determines this crossover .
	manualset3
144790	5	409253	5	NULL	NULL	0	NULL	crossover 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration dependence gives evidence that the Coulomb interaction energy is the energy scale that determines this crossover .
	manualset3
144791	1	409254	5	NULL	NULL	0	NULL	concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of GSH increased further with a higher , toxic dose of HgCl2 ( 2.0-mumol / kg ) .
	manualset3
144792	2	409254	5	NULL	NULL	0	NULL	GSH 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of GSH increased further with a higher , toxic dose of HgCl2 ( 2.0-mumol / kg ) .
	manualset3
144793	3	409254	5	NULL	NULL	0	NULL	dose 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of GSH increased further with a higher , toxic dose of HgCl2 ( 2.0-mumol / kg ) .
	manualset3
144794	4	409254	5	NULL	NULL	0	NULL	HgCl2 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of GSH increased further with a higher , toxic dose of HgCl2 ( 2.0-mumol / kg ) .
	manualset3
144795	5	409254	5	NULL	NULL	0	NULL	2.0-mumol / kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of GSH increased further with a higher , toxic dose of HgCl2 ( 2.0-mumol / kg ) .
	manualset3
144796	1	409255	5	NULL	NULL	0	NULL	concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of bupivacaine in patients determined by this method agreed well with the values obtained from an alternative method , making the technique applicable for pharmacokinetic studies in humans .
	manualset3
144797	2	409255	5	NULL	NULL	0	NULL	bupivacaine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of bupivacaine in patients determined by this method agreed well with the values obtained from an alternative method , making the technique applicable for pharmacokinetic studies in humans .
	manualset3
144798	3	409255	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of bupivacaine in patients determined by this method agreed well with the values obtained from an alternative method , making the technique applicable for pharmacokinetic studies in humans .
	manualset3
144799	4	409255	5	NULL	NULL	0	NULL	method 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of bupivacaine in patients determined by this method agreed well with the values obtained from an alternative method , making the technique applicable for pharmacokinetic studies in humans .
	manualset3
144800	5	409255	5	NULL	NULL	0	NULL	values 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of bupivacaine in patients determined by this method agreed well with the values obtained from an alternative method , making the technique applicable for pharmacokinetic studies in humans .
	manualset3
144801	6	409255	5	NULL	NULL	0	NULL	alternative method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of bupivacaine in patients determined by this method agreed well with the values obtained from an alternative method , making the technique applicable for pharmacokinetic studies in humans .
	manualset3
144802	7	409255	5	NULL	NULL	0	NULL	technique 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of bupivacaine in patients determined by this method agreed well with the values obtained from an alternative method , making the technique applicable for pharmacokinetic studies in humans .
	manualset3
144803	8	409255	5	NULL	NULL	0	NULL	pharmacokinetic studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of bupivacaine in patients determined by this method agreed well with the values obtained from an alternative method , making the technique applicable for pharmacokinetic studies in humans .
	manualset3
144804	9	409255	5	NULL	NULL	0	NULL	humans 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of bupivacaine in patients determined by this method agreed well with the values obtained from an alternative method , making the technique applicable for pharmacokinetic studies in humans .
	manualset3
144805	1	409256	5	NULL	NULL	0	NULL	concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of clathrin heavy-chain protein was the same in cells grown in liquid media ( high rates of pinocytosis ) as in cells grown with bacteria ( low rates of pinocytosis ) , which suggests that regulation of pinocytosis in these cells is not achieved by altering the concentration of clathrin .
	manualset3
144806	2	409256	5	NULL	NULL	0	NULL	clathrin heavy-chain protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of clathrin heavy-chain protein was the same in cells grown in liquid media ( high rates of pinocytosis ) as in cells grown with bacteria ( low rates of pinocytosis ) , which suggests that regulation of pinocytosis in these cells is not achieved by altering the concentration of clathrin .
	manualset3
144807	3	409256	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of clathrin heavy-chain protein was the same in cells grown in liquid media ( high rates of pinocytosis ) as in cells grown with bacteria ( low rates of pinocytosis ) , which suggests that regulation of pinocytosis in these cells is not achieved by altering the concentration of clathrin .
	manualset3
144808	4	409256	5	NULL	NULL	0	NULL	liquid media	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of clathrin heavy-chain protein was the same in cells grown in liquid media ( high rates of pinocytosis ) as in cells grown with bacteria ( low rates of pinocytosis ) , which suggests that regulation of pinocytosis in these cells is not achieved by altering the concentration of clathrin .
	manualset3
144809	5	409256	5	NULL	NULL	0	NULL	high rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of clathrin heavy-chain protein was the same in cells grown in liquid media ( high rates of pinocytosis ) as in cells grown with bacteria ( low rates of pinocytosis ) , which suggests that regulation of pinocytosis in these cells is not achieved by altering the concentration of clathrin .
	manualset3
144810	6	409256	5	NULL	NULL	0	NULL	pinocytosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of clathrin heavy-chain protein was the same in cells grown in liquid media ( high rates of pinocytosis ) as in cells grown with bacteria ( low rates of pinocytosis ) , which suggests that regulation of pinocytosis in these cells is not achieved by altering the concentration of clathrin .
	manualset3
144811	7	409256	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of clathrin heavy-chain protein was the same in cells grown in liquid media ( high rates of pinocytosis ) as in cells grown with bacteria ( low rates of pinocytosis ) , which suggests that regulation of pinocytosis in these cells is not achieved by altering the concentration of clathrin .
	manualset3
144812	8	409256	5	NULL	NULL	0	NULL	bacteria 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of clathrin heavy-chain protein was the same in cells grown in liquid media ( high rates of pinocytosis ) as in cells grown with bacteria ( low rates of pinocytosis ) , which suggests that regulation of pinocytosis in these cells is not achieved by altering the concentration of clathrin .
	manualset3
144813	9	409256	5	NULL	NULL	0	NULL	low rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of clathrin heavy-chain protein was the same in cells grown in liquid media ( high rates of pinocytosis ) as in cells grown with bacteria ( low rates of pinocytosis ) , which suggests that regulation of pinocytosis in these cells is not achieved by altering the concentration of clathrin .
	manualset3
144814	10	409256	5	NULL	NULL	0	NULL	pinocytosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of clathrin heavy-chain protein was the same in cells grown in liquid media ( high rates of pinocytosis ) as in cells grown with bacteria ( low rates of pinocytosis ) , which suggests that regulation of pinocytosis in these cells is not achieved by altering the concentration of clathrin .
	manualset3
144815	11	409256	5	NULL	NULL	0	NULL	regulation of pinocytosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of clathrin heavy-chain protein was the same in cells grown in liquid media ( high rates of pinocytosis ) as in cells grown with bacteria ( low rates of pinocytosis ) , which suggests that regulation of pinocytosis in these cells is not achieved by altering the concentration of clathrin .
	manualset3
144816	12	409256	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of clathrin heavy-chain protein was the same in cells grown in liquid media ( high rates of pinocytosis ) as in cells grown with bacteria ( low rates of pinocytosis ) , which suggests that regulation of pinocytosis in these cells is not achieved by altering the concentration of clathrin .
	manualset3
144817	13	409256	5	NULL	NULL	0	NULL	concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of clathrin heavy-chain protein was the same in cells grown in liquid media ( high rates of pinocytosis ) as in cells grown with bacteria ( low rates of pinocytosis ) , which suggests that regulation of pinocytosis in these cells is not achieved by altering the concentration of clathrin .
	manualset3
144818	14	409256	5	NULL	NULL	0	NULL	clathrin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of clathrin heavy-chain protein was the same in cells grown in liquid media ( high rates of pinocytosis ) as in cells grown with bacteria ( low rates of pinocytosis ) , which suggests that regulation of pinocytosis in these cells is not achieved by altering the concentration of clathrin .
	manualset3
144819	1	409257	5	NULL	NULL	0	NULL	concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of copper in plasma and that of lead in hair were higher in hypertensive subjects than in normotensives , but the concentrations of zinc , magnesium and selenium in plasma , urine and hair were similar to those of normotensives .
	manualset3
144820	2	409257	5	NULL	NULL	0	NULL	copper 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of copper in plasma and that of lead in hair were higher in hypertensive subjects than in normotensives , but the concentrations of zinc , magnesium and selenium in plasma , urine and hair were similar to those of normotensives .
	manualset3
144821	3	409257	5	NULL	NULL	0	NULL	plasma 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of copper in plasma and that of lead in hair were higher in hypertensive subjects than in normotensives , but the concentrations of zinc , magnesium and selenium in plasma , urine and hair were similar to those of normotensives .
	manualset3
144822	4	409257	5	NULL	NULL	0	NULL	lead 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of copper in plasma and that of lead in hair were higher in hypertensive subjects than in normotensives , but the concentrations of zinc , magnesium and selenium in plasma , urine and hair were similar to those of normotensives .
	manualset3
144823	5	409257	5	NULL	NULL	0	NULL	hair 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of copper in plasma and that of lead in hair were higher in hypertensive subjects than in normotensives , but the concentrations of zinc , magnesium and selenium in plasma , urine and hair were similar to those of normotensives .
	manualset3
144824	6	409257	5	NULL	NULL	NULL	NULL	hypertensive subjects 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The concentration of copper in plasma and that of lead in hair were higher in hypertensive subjects than in normotensives , but the concentrations of zinc , magnesium and selenium in plasma , urine and hair were similar to those of normotensives .
	manualset3
144825	7	409257	5	NULL	NULL	NULL	NULL	normotensives 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The concentration of copper in plasma and that of lead in hair were higher in hypertensive subjects than in normotensives , but the concentrations of zinc , magnesium and selenium in plasma , urine and hair were similar to those of normotensives .
	manualset3
144826	8	409257	5	NULL	NULL	0	NULL	concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of copper in plasma and that of lead in hair were higher in hypertensive subjects than in normotensives , but the concentrations of zinc , magnesium and selenium in plasma , urine and hair were similar to those of normotensives .
	manualset3
144827	9	409257	5	NULL	NULL	0	NULL	zinc 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of copper in plasma and that of lead in hair were higher in hypertensive subjects than in normotensives , but the concentrations of zinc , magnesium and selenium in plasma , urine and hair were similar to those of normotensives .
	manualset3
144828	10	409257	5	NULL	NULL	0	NULL	magnesium 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of copper in plasma and that of lead in hair were higher in hypertensive subjects than in normotensives , but the concentrations of zinc , magnesium and selenium in plasma , urine and hair were similar to those of normotensives .
	manualset3
144829	11	409257	5	NULL	NULL	0	NULL	selenium 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of copper in plasma and that of lead in hair were higher in hypertensive subjects than in normotensives , but the concentrations of zinc , magnesium and selenium in plasma , urine and hair were similar to those of normotensives .
	manualset3
144830	12	409257	5	NULL	NULL	0	NULL	plasma 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of copper in plasma and that of lead in hair were higher in hypertensive subjects than in normotensives , but the concentrations of zinc , magnesium and selenium in plasma , urine and hair were similar to those of normotensives .
	manualset3
144831	13	409257	5	NULL	NULL	0	NULL	urine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of copper in plasma and that of lead in hair were higher in hypertensive subjects than in normotensives , but the concentrations of zinc , magnesium and selenium in plasma , urine and hair were similar to those of normotensives .
	manualset3
144832	14	409257	5	NULL	NULL	0	NULL	hair 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of copper in plasma and that of lead in hair were higher in hypertensive subjects than in normotensives , but the concentrations of zinc , magnesium and selenium in plasma , urine and hair were similar to those of normotensives .
	manualset3
144833	15	409257	5	NULL	NULL	NULL	NULL	normotensives 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The concentration of copper in plasma and that of lead in hair were higher in hypertensive subjects than in normotensives , but the concentrations of zinc , magnesium and selenium in plasma , urine and hair were similar to those of normotensives .
	manualset3
144834	1	409258	5	NULL	NULL	0	NULL	concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of free disopyramide decreased as the pH was increased from 7.0 to 7.8 .
	manualset3
144846	2	409258	5	NULL	NULL	0	NULL	disopyramide 	dr												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of free disopyramide decreased as the pH was increased from 7.0 to 7.8 .
	manualset3
144847	3	409258	5	NULL	NULL	0	NULL	pH 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of free disopyramide decreased as the pH was increased from 7.0 to 7.8 .
	manualset3
144848	4	409258	5	NULL	NULL	0	NULL	7.0 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of free disopyramide decreased as the pH was increased from 7.0 to 7.8 .
	manualset3
144849	5	409258	5	NULL	NULL	0	NULL	7.8	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of free disopyramide decreased as the pH was increased from 7.0 to 7.8 .
	manualset3
144850	1	409259	5	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant increase in gene expression of muscarinic M3 , 7 nicotinic acetylcholine , insulin , Vitamin D receptors , acetylcholine esterase , choline acetyl transferase and GLUT 3 were observed in the brainstem of diabetic rats .
	manualset3
144851	2	409259	5	NULL	NULL	0	NULL	gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant increase in gene expression of muscarinic M3 , 7 nicotinic acetylcholine , insulin , Vitamin D receptors , acetylcholine esterase , choline acetyl transferase and GLUT 3 were observed in the brainstem of diabetic rats .
	manualset3
144852	3	409259	5	NULL	NULL	0	NULL	muscarinic M3 receptor	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant increase in gene expression of muscarinic M3 , 7 nicotinic acetylcholine , insulin , Vitamin D receptors , acetylcholine esterase , choline acetyl transferase and GLUT 3 were observed in the brainstem of diabetic rats .
	manualset3
144853	4	409259	5	NULL	NULL	0	NULL	7 nicotinic acetylcholine receptor	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant increase in gene expression of muscarinic M3 , 7 nicotinic acetylcholine , insulin , Vitamin D receptors , acetylcholine esterase , choline acetyl transferase and GLUT 3 were observed in the brainstem of diabetic rats .
	manualset3
144854	5	409259	5	NULL	NULL	0	NULL	insulin receptor	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant increase in gene expression of muscarinic M3 , 7 nicotinic acetylcholine , insulin , Vitamin D receptors , acetylcholine esterase , choline acetyl transferase and GLUT 3 were observed in the brainstem of diabetic rats .
	manualset3
144855	6	409259	5	NULL	NULL	0	NULL	Vitamin D receptor	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant increase in gene expression of muscarinic M3 , 7 nicotinic acetylcholine , insulin , Vitamin D receptors , acetylcholine esterase , choline acetyl transferase and GLUT 3 were observed in the brainstem of diabetic rats .
	manualset3
144856	7	409259	5	NULL	NULL	NULL	NULL	acetylcholine esterase	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A significant increase in gene expression of muscarinic M3 , 7 nicotinic acetylcholine , insulin , Vitamin D receptors , acetylcholine esterase , choline acetyl transferase and GLUT 3 were observed in the brainstem of diabetic rats .
	manualset3
144857	8	409259	5	NULL	NULL	0	NULL	choline acetyl transferase	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant increase in gene expression of muscarinic M3 , 7 nicotinic acetylcholine , insulin , Vitamin D receptors , acetylcholine esterase , choline acetyl transferase and GLUT 3 were observed in the brainstem of diabetic rats .
	manualset3
144858	9	409259	5	NULL	NULL	0	NULL	GLUT 3	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant increase in gene expression of muscarinic M3 , 7 nicotinic acetylcholine , insulin , Vitamin D receptors , acetylcholine esterase , choline acetyl transferase and GLUT 3 were observed in the brainstem of diabetic rats .
	manualset3
144859	10	409259	5	NULL	NULL	0	NULL	brainstem 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant increase in gene expression of muscarinic M3 , 7 nicotinic acetylcholine , insulin , Vitamin D receptors , acetylcholine esterase , choline acetyl transferase and GLUT 3 were observed in the brainstem of diabetic rats .
	manualset3
144860	11	409259	5	NULL	NULL	0	NULL	diabetic rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant increase in gene expression of muscarinic M3 , 7 nicotinic acetylcholine , insulin , Vitamin D receptors , acetylcholine esterase , choline acetyl transferase and GLUT 3 were observed in the brainstem of diabetic rats .
	manualset3
144861	1	409260	5	NULL	NULL	0	NULL	concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of peptide required for 50 % inhibition of FVIII activity ( IC50 ) was reduced for the I566T ( 800 mumol/L ) and the S558F ( 960 mumol/L ) mutants compared with wild-type FVIII ( ) 2 , 000 mumol/L ) .
	manualset3
144862	2	409260	5	NULL	NULL	0	NULL	peptide 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of peptide required for 50 % inhibition of FVIII activity ( IC50 ) was reduced for the I566T ( 800 mumol/L ) and the S558F ( 960 mumol/L ) mutants compared with wild-type FVIII ( ) 2 , 000 mumol/L ) .
	manualset3
144863	3	409260	5	NULL	NULL	0	NULL	50 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of peptide required for 50 % inhibition of FVIII activity ( IC50 ) was reduced for the I566T ( 800 mumol/L ) and the S558F ( 960 mumol/L ) mutants compared with wild-type FVIII ( ) 2 , 000 mumol/L ) .
	manualset3
144864	4	409260	5	NULL	NULL	0	NULL	inhibition 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of peptide required for 50 % inhibition of FVIII activity ( IC50 ) was reduced for the I566T ( 800 mumol/L ) and the S558F ( 960 mumol/L ) mutants compared with wild-type FVIII ( ) 2 , 000 mumol/L ) .
	manualset3
144865	5	409260	5	NULL	NULL	0	NULL	FVIII activity ( IC50 )	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of peptide required for 50 % inhibition of FVIII activity ( IC50 ) was reduced for the I566T ( 800 mumol/L ) and the S558F ( 960 mumol/L ) mutants compared with wild-type FVIII ( ) 2 , 000 mumol/L ) .
	manualset3
144866	6	409260	5	NULL	NULL	NULL	NULL	I566T mutants	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The concentration of peptide required for 50 % inhibition of FVIII activity ( IC50 ) was reduced for the I566T ( 800 mumol/L ) and the S558F ( 960 mumol/L ) mutants compared with wild-type FVIII ( ) 2 , 000 mumol/L ) .
	manualset3
144867	7	409260	5	NULL	NULL	0	NULL	800 mumol/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of peptide required for 50 % inhibition of FVIII activity ( IC50 ) was reduced for the I566T ( 800 mumol/L ) and the S558F ( 960 mumol/L ) mutants compared with wild-type FVIII ( ) 2 , 000 mumol/L ) .
	manualset3
144868	8	409260	5	NULL	NULL	NULL	NULL	S558F mutants	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The concentration of peptide required for 50 % inhibition of FVIII activity ( IC50 ) was reduced for the I566T ( 800 mumol/L ) and the S558F ( 960 mumol/L ) mutants compared with wild-type FVIII ( ) 2 , 000 mumol/L ) .
	manualset3
144869	9	409260	5	NULL	NULL	0	NULL	960 mumol/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of peptide required for 50 % inhibition of FVIII activity ( IC50 ) was reduced for the I566T ( 800 mumol/L ) and the S558F ( 960 mumol/L ) mutants compared with wild-type FVIII ( ) 2 , 000 mumol/L ) .
	manualset3
144870	10	409260	5	NULL	NULL	0	NULL	wild-type FVIII	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of peptide required for 50 % inhibition of FVIII activity ( IC50 ) was reduced for the I566T ( 800 mumol/L ) and the S558F ( 960 mumol/L ) mutants compared with wild-type FVIII ( ) 2 , 000 mumol/L ) .
	manualset3
144871	11	409260	5	NULL	NULL	0	NULL	2 , 000 mumol/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of peptide required for 50 % inhibition of FVIII activity ( IC50 ) was reduced for the I566T ( 800 mumol/L ) and the S558F ( 960 mumol/L ) mutants compared with wild-type FVIII ( ) 2 , 000 mumol/L ) .
	manualset3
144872	1	409261	5	NULL	NULL	0	NULL	concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of pyrrolidone carboxylate and gamma-glutamyl amino acids , intermediates of the gamma-glutamyl cycle , was determined by a gas chromatographic procedure coupled with electron capture detection .
	manualset3
144873	2	409261	5	NULL	NULL	0	NULL	pyrrolidone carboxylate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of pyrrolidone carboxylate and gamma-glutamyl amino acids , intermediates of the gamma-glutamyl cycle , was determined by a gas chromatographic procedure coupled with electron capture detection .
	manualset3
144874	3	409261	5	NULL	NULL	0	NULL	gamma-glutamyl amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of pyrrolidone carboxylate and gamma-glutamyl amino acids , intermediates of the gamma-glutamyl cycle , was determined by a gas chromatographic procedure coupled with electron capture detection .
	manualset3
144875	4	409261	5	NULL	NULL	0	NULL	intermediates of the gamma-glutamyl cycle	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of pyrrolidone carboxylate and gamma-glutamyl amino acids , intermediates of the gamma-glutamyl cycle , was determined by a gas chromatographic procedure coupled with electron capture detection .
	manualset3
144876	5	409261	5	NULL	NULL	0	NULL	gas chromatographic procedure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of pyrrolidone carboxylate and gamma-glutamyl amino acids , intermediates of the gamma-glutamyl cycle , was determined by a gas chromatographic procedure coupled with electron capture detection .
	manualset3
144877	6	409261	5	NULL	NULL	0	NULL	electron capture detection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of pyrrolidone carboxylate and gamma-glutamyl amino acids , intermediates of the gamma-glutamyl cycle , was determined by a gas chromatographic procedure coupled with electron capture detection .
	manualset3
144878	1	409262	5	NULL	NULL	0	NULL	concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of quinaldate required to cause a 50-per-cent inhibition of ADP-activated oxygen uptake slightly differs with various substrates in the same type of mitochondria , and differs with the same substrate in the case of the two types of mitochondria and lies within the mM order of magnitude .
	manualset3
144879	2	409262	5	NULL	NULL	0	NULL	quinaldate 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of quinaldate required to cause a 50-per-cent inhibition of ADP-activated oxygen uptake slightly differs with various substrates in the same type of mitochondria , and differs with the same substrate in the case of the two types of mitochondria and lies within the mM order of magnitude .
	manualset3
144881	4	409262	5	NULL	NULL	0	NULL	50-per-cent inhibition	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of quinaldate required to cause a 50-per-cent inhibition of ADP-activated oxygen uptake slightly differs with various substrates in the same type of mitochondria , and differs with the same substrate in the case of the two types of mitochondria and lies within the mM order of magnitude .
	manualset3
144882	5	409262	5	NULL	NULL	0	NULL	inhibition 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of quinaldate required to cause a 50-per-cent inhibition of ADP-activated oxygen uptake slightly differs with various substrates in the same type of mitochondria , and differs with the same substrate in the case of the two types of mitochondria and lies within the mM order of magnitude .
	manualset3
144883	6	409262	5	NULL	NULL	0	NULL	ADP-activated oxygen uptake	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of quinaldate required to cause a 50-per-cent inhibition of ADP-activated oxygen uptake slightly differs with various substrates in the same type of mitochondria , and differs with the same substrate in the case of the two types of mitochondria and lies within the mM order of magnitude .
	manualset3
144884	7	409262	5	NULL	NULL	0	NULL	substrates 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of quinaldate required to cause a 50-per-cent inhibition of ADP-activated oxygen uptake slightly differs with various substrates in the same type of mitochondria , and differs with the same substrate in the case of the two types of mitochondria and lies within the mM order of magnitude .
	manualset3
144885	8	409262	5	NULL	NULL	0	NULL	mitochondria 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of quinaldate required to cause a 50-per-cent inhibition of ADP-activated oxygen uptake slightly differs with various substrates in the same type of mitochondria , and differs with the same substrate in the case of the two types of mitochondria and lies within the mM order of magnitude .
	manualset3
144886	9	409262	5	NULL	NULL	0	NULL	substrate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of quinaldate required to cause a 50-per-cent inhibition of ADP-activated oxygen uptake slightly differs with various substrates in the same type of mitochondria , and differs with the same substrate in the case of the two types of mitochondria and lies within the mM order of magnitude .
	manualset3
144887	10	409262	5	NULL	NULL	0	NULL	two types	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of quinaldate required to cause a 50-per-cent inhibition of ADP-activated oxygen uptake slightly differs with various substrates in the same type of mitochondria , and differs with the same substrate in the case of the two types of mitochondria and lies within the mM order of magnitude .
	manualset3
144889	11	409262	5	NULL	NULL	0	NULL	mitochondria 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of quinaldate required to cause a 50-per-cent inhibition of ADP-activated oxygen uptake slightly differs with various substrates in the same type of mitochondria , and differs with the same substrate in the case of the two types of mitochondria and lies within the mM order of magnitude .
	manualset3
144890	12	409262	5	NULL	NULL	0	NULL	mM order of magnitude	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of quinaldate required to cause a 50-per-cent inhibition of ADP-activated oxygen uptake slightly differs with various substrates in the same type of mitochondria , and differs with the same substrate in the case of the two types of mitochondria and lies within the mM order of magnitude .
	manualset3
144891	13	409262	5	NULL	NULL	0	NULL	type 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentration of quinaldate required to cause a 50-per-cent inhibition of ADP-activated oxygen uptake slightly differs with various substrates in the same type of mitochondria , and differs with the same substrate in the case of the two types of mitochondria and lies within the mM order of magnitude .
	manualset3
144892	1	409263	5	NULL	NULL	0	NULL	concentrations ( femtomoles/mg protein ( fmol/mg protein ) ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations ( femtomoles/mg protein ( fmol/mg protein ) ) and affinities of unoccupied LH/hCG binding sites were characterized in all samples of myometrium .
	manualset3
144893	2	409263	5	NULL	NULL	0	NULL	affinities 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations ( femtomoles/mg protein ( fmol/mg protein ) ) and affinities of unoccupied LH/hCG binding sites were characterized in all samples of myometrium .
	manualset3
144894	3	409263	5	NULL	NULL	0	NULL	unoccupied LH/hCG binding sites	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations ( femtomoles/mg protein ( fmol/mg protein ) ) and affinities of unoccupied LH/hCG binding sites were characterized in all samples of myometrium .
	manualset3
144895	4	409263	5	NULL	NULL	0	NULL	samples 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations ( femtomoles/mg protein ( fmol/mg protein ) ) and affinities of unoccupied LH/hCG binding sites were characterized in all samples of myometrium .
	manualset3
144896	5	409263	5	NULL	NULL	0	NULL	myometrium 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations ( femtomoles/mg protein ( fmol/mg protein ) ) and affinities of unoccupied LH/hCG binding sites were characterized in all samples of myometrium .
	manualset3
144897	1	409264	5	NULL	NULL	0	NULL	concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations of the proteins examined were not significantly altered by repeated freeze-thaw cycles , nor by extended clotting times at 4 degrees C or 20 degrees C. We conclude that serum samples for the determination of IL-6 , sIL-6R and CC16 can be stored at -20 degrees C for several years , but for IL-10 determinations , storage at -70 degrees C is recommended .
	manualset3
144898	2	409264	5	NULL	NULL	0	NULL	proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations of the proteins examined were not significantly altered by repeated freeze-thaw cycles , nor by extended clotting times at 4 degrees C or 20 degrees C. We conclude that serum samples for the determination of IL-6 , sIL-6R and CC16 can be stored at -20 degrees C for several years , but for IL-10 determinations , storage at -70 degrees C is recommended .
	manualset3
144899	3	409264	5	NULL	NULL	0	NULL	repeated freeze-thaw cycles	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations of the proteins examined were not significantly altered by repeated freeze-thaw cycles , nor by extended clotting times at 4 degrees C or 20 degrees C. We conclude that serum samples for the determination of IL-6 , sIL-6R and CC16 can be stored at -20 degrees C for several years , but for IL-10 determinations , storage at -70 degrees C is recommended .
	manualset3
144900	4	409264	5	NULL	NULL	0	NULL	extended clotting times	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations of the proteins examined were not significantly altered by repeated freeze-thaw cycles , nor by extended clotting times at 4 degrees C or 20 degrees C. We conclude that serum samples for the determination of IL-6 , sIL-6R and CC16 can be stored at -20 degrees C for several years , but for IL-10 determinations , storage at -70 degrees C is recommended .
	manualset3
144901	5	409264	5	NULL	NULL	0	NULL	4 degrees C or 20 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations of the proteins examined were not significantly altered by repeated freeze-thaw cycles , nor by extended clotting times at 4 degrees C or 20 degrees C. We conclude that serum samples for the determination of IL-6 , sIL-6R and CC16 can be stored at -20 degrees C for several years , but for IL-10 determinations , storage at -70 degrees C is recommended .
	manualset3
144902	6	409264	5	NULL	NULL	0	NULL	serum samples	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations of the proteins examined were not significantly altered by repeated freeze-thaw cycles , nor by extended clotting times at 4 degrees C or 20 degrees C. We conclude that serum samples for the determination of IL-6 , sIL-6R and CC16 can be stored at -20 degrees C for several years , but for IL-10 determinations , storage at -70 degrees C is recommended .
	manualset3
144903	7	409264	5	NULL	NULL	0	NULL	determination 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations of the proteins examined were not significantly altered by repeated freeze-thaw cycles , nor by extended clotting times at 4 degrees C or 20 degrees C. We conclude that serum samples for the determination of IL-6 , sIL-6R and CC16 can be stored at -20 degrees C for several years , but for IL-10 determinations , storage at -70 degrees C is recommended .
	manualset3
144904	8	409264	5	NULL	NULL	0	NULL	IL-6 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations of the proteins examined were not significantly altered by repeated freeze-thaw cycles , nor by extended clotting times at 4 degrees C or 20 degrees C. We conclude that serum samples for the determination of IL-6 , sIL-6R and CC16 can be stored at -20 degrees C for several years , but for IL-10 determinations , storage at -70 degrees C is recommended .
	manualset3
144905	9	409264	5	NULL	NULL	0	NULL	sIL-6R 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations of the proteins examined were not significantly altered by repeated freeze-thaw cycles , nor by extended clotting times at 4 degrees C or 20 degrees C. We conclude that serum samples for the determination of IL-6 , sIL-6R and CC16 can be stored at -20 degrees C for several years , but for IL-10 determinations , storage at -70 degrees C is recommended .
	manualset3
144906	10	409264	5	NULL	NULL	0	NULL	CC16 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations of the proteins examined were not significantly altered by repeated freeze-thaw cycles , nor by extended clotting times at 4 degrees C or 20 degrees C. We conclude that serum samples for the determination of IL-6 , sIL-6R and CC16 can be stored at -20 degrees C for several years , but for IL-10 determinations , storage at -70 degrees C is recommended .
	manualset3
144907	11	409264	5	NULL	NULL	0	NULL	-20 degrees C 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations of the proteins examined were not significantly altered by repeated freeze-thaw cycles , nor by extended clotting times at 4 degrees C or 20 degrees C. We conclude that serum samples for the determination of IL-6 , sIL-6R and CC16 can be stored at -20 degrees C for several years , but for IL-10 determinations , storage at -70 degrees C is recommended .
	manualset3
144908	12	409264	5	NULL	NULL	0	NULL	several years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations of the proteins examined were not significantly altered by repeated freeze-thaw cycles , nor by extended clotting times at 4 degrees C or 20 degrees C. We conclude that serum samples for the determination of IL-6 , sIL-6R and CC16 can be stored at -20 degrees C for several years , but for IL-10 determinations , storage at -70 degrees C is recommended .
	manualset3
144909	13	409264	5	NULL	NULL	0	NULL	 IL-10 determinations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations of the proteins examined were not significantly altered by repeated freeze-thaw cycles , nor by extended clotting times at 4 degrees C or 20 degrees C. We conclude that serum samples for the determination of IL-6 , sIL-6R and CC16 can be stored at -20 degrees C for several years , but for IL-10 determinations , storage at -70 degrees C is recommended .
	manualset3
144910	14	409264	5	NULL	NULL	0	NULL	storage 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations of the proteins examined were not significantly altered by repeated freeze-thaw cycles , nor by extended clotting times at 4 degrees C or 20 degrees C. We conclude that serum samples for the determination of IL-6 , sIL-6R and CC16 can be stored at -20 degrees C for several years , but for IL-10 determinations , storage at -70 degrees C is recommended .
	manualset3
144911	15	409264	5	NULL	NULL	0	NULL	 -70 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations of the proteins examined were not significantly altered by repeated freeze-thaw cycles , nor by extended clotting times at 4 degrees C or 20 degrees C. We conclude that serum samples for the determination of IL-6 , sIL-6R and CC16 can be stored at -20 degrees C for several years , but for IL-10 determinations , storage at -70 degrees C is recommended .
	manualset3
144912	1	409265	5	NULL	NULL	0	NULL	concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations of total radioactivity , conjugated estriol metabolites , estriol , estriol-o-glucosiduronate , estriol-16alpha-glucosiduronate , estriol-3-sulfate and estriol-3-sulfate , 16alpha-glucosiduronate were determined in plasma from the femoral artery ( A ) , hepatic vein ( HV ) and superior mesenteric vein ( SMV ) .
	manualset3
144913	2	409265	5	NULL	NULL	0	NULL	radioactivity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations of total radioactivity , conjugated estriol metabolites , estriol , estriol-o-glucosiduronate , estriol-16alpha-glucosiduronate , estriol-3-sulfate and estriol-3-sulfate , 16alpha-glucosiduronate were determined in plasma from the femoral artery ( A ) , hepatic vein ( HV ) and superior mesenteric vein ( SMV ) .
	manualset3
144914	3	409265	5	NULL	NULL	0	NULL	conjugated estriol metabolites	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations of total radioactivity , conjugated estriol metabolites , estriol , estriol-o-glucosiduronate , estriol-16alpha-glucosiduronate , estriol-3-sulfate and estriol-3-sulfate , 16alpha-glucosiduronate were determined in plasma from the femoral artery ( A ) , hepatic vein ( HV ) and superior mesenteric vein ( SMV ) .
	manualset3
144915	4	409265	5	NULL	NULL	0	NULL	estriol 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations of total radioactivity , conjugated estriol metabolites , estriol , estriol-o-glucosiduronate , estriol-16alpha-glucosiduronate , estriol-3-sulfate and estriol-3-sulfate , 16alpha-glucosiduronate were determined in plasma from the femoral artery ( A ) , hepatic vein ( HV ) and superior mesenteric vein ( SMV ) .
	manualset3
144916	5	409265	5	NULL	NULL	0	NULL	estriol-o-glucosiduronate 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations of total radioactivity , conjugated estriol metabolites , estriol , estriol-o-glucosiduronate , estriol-16alpha-glucosiduronate , estriol-3-sulfate and estriol-3-sulfate , 16alpha-glucosiduronate were determined in plasma from the femoral artery ( A ) , hepatic vein ( HV ) and superior mesenteric vein ( SMV ) .
	manualset3
144917	6	409265	5	NULL	NULL	0	NULL	estriol-16alpha-glucosiduronate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations of total radioactivity , conjugated estriol metabolites , estriol , estriol-o-glucosiduronate , estriol-16alpha-glucosiduronate , estriol-3-sulfate and estriol-3-sulfate , 16alpha-glucosiduronate were determined in plasma from the femoral artery ( A ) , hepatic vein ( HV ) and superior mesenteric vein ( SMV ) .
	manualset3
144918	7	409265	5	NULL	NULL	0	NULL	estriol-3-sulfate and estriol-3-sulfate 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations of total radioactivity , conjugated estriol metabolites , estriol , estriol-o-glucosiduronate , estriol-16alpha-glucosiduronate , estriol-3-sulfate and estriol-3-sulfate , 16alpha-glucosiduronate were determined in plasma from the femoral artery ( A ) , hepatic vein ( HV ) and superior mesenteric vein ( SMV ) .
	manualset3
144919	8	409265	5	NULL	NULL	0	NULL	16alpha-glucosiduronate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations of total radioactivity , conjugated estriol metabolites , estriol , estriol-o-glucosiduronate , estriol-16alpha-glucosiduronate , estriol-3-sulfate and estriol-3-sulfate , 16alpha-glucosiduronate were determined in plasma from the femoral artery ( A ) , hepatic vein ( HV ) and superior mesenteric vein ( SMV ) .
	manualset3
144920	9	409265	5	NULL	NULL	0	NULL	plasma 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations of total radioactivity , conjugated estriol metabolites , estriol , estriol-o-glucosiduronate , estriol-16alpha-glucosiduronate , estriol-3-sulfate and estriol-3-sulfate , 16alpha-glucosiduronate were determined in plasma from the femoral artery ( A ) , hepatic vein ( HV ) and superior mesenteric vein ( SMV ) .
	manualset3
144921	10	409265	5	NULL	NULL	0	NULL	femoral artery ( A )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations of total radioactivity , conjugated estriol metabolites , estriol , estriol-o-glucosiduronate , estriol-16alpha-glucosiduronate , estriol-3-sulfate and estriol-3-sulfate , 16alpha-glucosiduronate were determined in plasma from the femoral artery ( A ) , hepatic vein ( HV ) and superior mesenteric vein ( SMV ) .
	manualset3
144922	11	409265	5	NULL	NULL	0	NULL	hepatic vein ( HV ) 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations of total radioactivity , conjugated estriol metabolites , estriol , estriol-o-glucosiduronate , estriol-16alpha-glucosiduronate , estriol-3-sulfate and estriol-3-sulfate , 16alpha-glucosiduronate were determined in plasma from the femoral artery ( A ) , hepatic vein ( HV ) and superior mesenteric vein ( SMV ) .
	manualset3
144923	12	409265	5	NULL	NULL	0	NULL	superior mesenteric vein ( SMV )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The concentrations of total radioactivity , conjugated estriol metabolites , estriol , estriol-o-glucosiduronate , estriol-16alpha-glucosiduronate , estriol-3-sulfate and estriol-3-sulfate , 16alpha-glucosiduronate were determined in plasma from the femoral artery ( A ) , hepatic vein ( HV ) and superior mesenteric vein ( SMV ) .
	manualset3
144924	1	409266	5	NULL	NULL	NULL	NULL	pharmacogenomics 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The concept of `` pharmacogenomics '' or `` pharmacogenetics '' promises to offer the ultimate in personalized medicine , and the renin-angiotensin system ( RAS ) is one of the most plausible candidates for the application of this approach in the area of hypertension .
	manualset3
144925	2	409266	5	NULL	NULL	NULL	NULL	pharmacogenetics 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The concept of `` pharmacogenomics '' or `` pharmacogenetics '' promises to offer the ultimate in personalized medicine , and the renin-angiotensin system ( RAS ) is one of the most plausible candidates for the application of this approach in the area of hypertension .
	manualset3
144926	3	409266	5	NULL	NULL	NULL	NULL	personalized medicine	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The concept of `` pharmacogenomics '' or `` pharmacogenetics '' promises to offer the ultimate in personalized medicine , and the renin-angiotensin system ( RAS ) is one of the most plausible candidates for the application of this approach in the area of hypertension .
	manualset3
144927	4	409266	5	NULL	NULL	NULL	NULL	renin-angiotensin system ( RAS )	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The concept of `` pharmacogenomics '' or `` pharmacogenetics '' promises to offer the ultimate in personalized medicine , and the renin-angiotensin system ( RAS ) is one of the most plausible candidates for the application of this approach in the area of hypertension .
	manualset3
144928	5	409266	5	NULL	NULL	0	NULL	one 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The concept of `` pharmacogenomics '' or `` pharmacogenetics '' promises to offer the ultimate in personalized medicine , and the renin-angiotensin system ( RAS ) is one of the most plausible candidates for the application of this approach in the area of hypertension .
	manualset3
144929	6	409266	5	NULL	NULL	0	NULL	candidates 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concept of `` pharmacogenomics '' or `` pharmacogenetics '' promises to offer the ultimate in personalized medicine , and the renin-angiotensin system ( RAS ) is one of the most plausible candidates for the application of this approach in the area of hypertension .
	manualset3
144930	7	409266	5	NULL	NULL	0	NULL	application 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The concept of `` pharmacogenomics '' or `` pharmacogenetics '' promises to offer the ultimate in personalized medicine , and the renin-angiotensin system ( RAS ) is one of the most plausible candidates for the application of this approach in the area of hypertension .
	manualset3
144931	8	409266	5	NULL	NULL	0	NULL	approach 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The concept of `` pharmacogenomics '' or `` pharmacogenetics '' promises to offer the ultimate in personalized medicine , and the renin-angiotensin system ( RAS ) is one of the most plausible candidates for the application of this approach in the area of hypertension .
	manualset3
144932	9	409266	5	NULL	NULL	0	NULL	area 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The concept of `` pharmacogenomics '' or `` pharmacogenetics '' promises to offer the ultimate in personalized medicine , and the renin-angiotensin system ( RAS ) is one of the most plausible candidates for the application of this approach in the area of hypertension .
	manualset3
144933	10	409266	5	NULL	NULL	0	NULL	hypertension 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The concept of `` pharmacogenomics '' or `` pharmacogenetics '' promises to offer the ultimate in personalized medicine , and the renin-angiotensin system ( RAS ) is one of the most plausible candidates for the application of this approach in the area of hypertension .
	manualset3
144934	1	409267	5	NULL	NULL	0	NULL	concept 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The concept of uncanny anxiety can be distinguished from other clinical entities such as anxiety states , depression , or mourning .
	manualset3
144935	2	409267	5	NULL	NULL	0	NULL	uncanny anxiety	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The concept of uncanny anxiety can be distinguished from other clinical entities such as anxiety states , depression , or mourning .
	manualset3
144936	3	409267	5	NULL	NULL	0	NULL	clinical entities 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The concept of uncanny anxiety can be distinguished from other clinical entities such as anxiety states , depression , or mourning .
	manualset3
144937	4	409267	5	NULL	NULL	NULL	NULL	anxiety states 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The concept of uncanny anxiety can be distinguished from other clinical entities such as anxiety states , depression , or mourning .
	manualset3
144938	5	409267	5	NULL	NULL	0	NULL	depression 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The concept of uncanny anxiety can be distinguished from other clinical entities such as anxiety states , depression , or mourning .
	manualset3
144939	6	409267	5	NULL	NULL	0	NULL	mourning 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The concept of uncanny anxiety can be distinguished from other clinical entities such as anxiety states , depression , or mourning .
	manualset3
144940	1	409268	5	NULL	NULL	0	NULL	conceptual progression	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The conceptual progression shows that current controversies have old roots and that failed percepts often resurface after seemingly having been put to rest by argument and evidence .
	manualset3
144941	2	409268	5	NULL	NULL	0	NULL	controversies 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The conceptual progression shows that current controversies have old roots and that failed percepts often resurface after seemingly having been put to rest by argument and evidence .
	manualset3
144942	3	409268	5	NULL	NULL	0	NULL	old roots 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The conceptual progression shows that current controversies have old roots and that failed percepts often resurface after seemingly having been put to rest by argument and evidence .
	manualset3
144943	4	409268	5	NULL	NULL	0	NULL	failed percepts 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The conceptual progression shows that current controversies have old roots and that failed percepts often resurface after seemingly having been put to rest by argument and evidence .
	manualset3
144944	5	409268	5	NULL	NULL	0	NULL	rest 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The conceptual progression shows that current controversies have old roots and that failed percepts often resurface after seemingly having been put to rest by argument and evidence .
	manualset3
144945	6	409268	5	NULL	NULL	0	NULL	argument 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The conceptual progression shows that current controversies have old roots and that failed percepts often resurface after seemingly having been put to rest by argument and evidence .
	manualset3
144946	7	409268	5	NULL	NULL	0	NULL	evidence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The conceptual progression shows that current controversies have old roots and that failed percepts often resurface after seemingly having been put to rest by argument and evidence .
	manualset3
144947	1	409269	5	NULL	NULL	0	NULL	significant linear dose trend	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant linear dose trend was also seen for time to 1 mm ST-segment depression at 24 hours after dosing .
	manualset3
144948	2	409269	5	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant linear dose trend was also seen for time to 1 mm ST-segment depression at 24 hours after dosing .
	manualset3
144949	3	409269	5	NULL	NULL	0	NULL	1 mm ST-segment depression	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant linear dose trend was also seen for time to 1 mm ST-segment depression at 24 hours after dosing .
	manualset3
144950	4	409269	5	NULL	NULL	0	NULL	24 hours 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant linear dose trend was also seen for time to 1 mm ST-segment depression at 24 hours after dosing .
	manualset3
144951	5	409269	5	NULL	NULL	0	NULL	dosing 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant linear dose trend was also seen for time to 1 mm ST-segment depression at 24 hours after dosing .
	manualset3
144952	1	409270	5	NULL	NULL	0	NULL	conclusion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The conclusion is that a problem so widespread is a candidate for prevention , and that the few trials in this direction should be augmented .
	manualset3
144953	2	409270	5	NULL	NULL	0	NULL	problem 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The conclusion is that a problem so widespread is a candidate for prevention , and that the few trials in this direction should be augmented .
	manualset3
144954	3	409270	5	NULL	NULL	0	NULL	candidate 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The conclusion is that a problem so widespread is a candidate for prevention , and that the few trials in this direction should be augmented .
	manualset3
144955	4	409270	5	NULL	NULL	0	NULL	prevention 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The conclusion is that a problem so widespread is a candidate for prevention , and that the few trials in this direction should be augmented .
	manualset3
144956	5	409270	5	NULL	NULL	0	NULL	few trials	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The conclusion is that a problem so widespread is a candidate for prevention , and that the few trials in this direction should be augmented .
	manualset3
144957	6	409270	5	NULL	NULL	0	NULL	direction 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The conclusion is that a problem so widespread is a candidate for prevention , and that the few trials in this direction should be augmented .
	manualset3
144958	1	409271	5	NULL	NULL	0	NULL	quercetin 's multiple bioactivities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The concurrent targeting of quercetin 's multiple bioactivities presents a potent chemopreventative strategy , but because bioavailability of quercetin is poor it will be necessary to develop quercetin analogs to maximize the full chemopreventative potential of the compound .
	manualset3
144959	2	409271	5	NULL	NULL	0	NULL	potent chemopreventative strategy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The concurrent targeting of quercetin 's multiple bioactivities presents a potent chemopreventative strategy , but because bioavailability of quercetin is poor it will be necessary to develop quercetin analogs to maximize the full chemopreventative potential of the compound .
	manualset3
144960	3	409271	5	NULL	NULL	0	NULL	bioavailability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The concurrent targeting of quercetin 's multiple bioactivities presents a potent chemopreventative strategy , but because bioavailability of quercetin is poor it will be necessary to develop quercetin analogs to maximize the full chemopreventative potential of the compound .
	manualset3
144961	4	409271	5	NULL	NULL	0	NULL	quercetin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The concurrent targeting of quercetin 's multiple bioactivities presents a potent chemopreventative strategy , but because bioavailability of quercetin is poor it will be necessary to develop quercetin analogs to maximize the full chemopreventative potential of the compound .
	manualset3
144962	5	409271	5	NULL	NULL	0	NULL	quercetin analogs	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The concurrent targeting of quercetin 's multiple bioactivities presents a potent chemopreventative strategy , but because bioavailability of quercetin is poor it will be necessary to develop quercetin analogs to maximize the full chemopreventative potential of the compound .
	manualset3
144963	6	409271	5	NULL	NULL	0	NULL	chemopreventative potential 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The concurrent targeting of quercetin 's multiple bioactivities presents a potent chemopreventative strategy , but because bioavailability of quercetin is poor it will be necessary to develop quercetin analogs to maximize the full chemopreventative potential of the compound .
	manualset3
144964	7	409271	5	NULL	NULL	0	NULL	compound 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The concurrent targeting of quercetin 's multiple bioactivities presents a potent chemopreventative strategy , but because bioavailability of quercetin is poor it will be necessary to develop quercetin analogs to maximize the full chemopreventative potential of the compound .
	manualset3
144965	1	409272	5	NULL	NULL	0	NULL	conditioning regimen	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The conditioning regimen consisted of fludarabine 30 mg/m ( 2 ) / day ( days -5 , -4 , -3 ) and 2 Gy TBI ( 0.07 Gy/min ; day 0 ) .
	manualset3
144966	2	409272	5	NULL	NULL	0	NULL	fludarabine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The conditioning regimen consisted of fludarabine 30 mg/m ( 2 ) / day ( days -5 , -4 , -3 ) and 2 Gy TBI ( 0.07 Gy/min ; day 0 ) .
	manualset3
144967	3	409272	5	NULL	NULL	0	NULL	30 mg/m ( 2 ) / day ( days -5 , -4 , -3 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The conditioning regimen consisted of fludarabine 30 mg/m ( 2 ) / day ( days -5 , -4 , -3 ) and 2 Gy TBI ( 0.07 Gy/min ; day 0 ) .
	manualset3
144968	4	409272	5	NULL	NULL	0	NULL	2 Gy TBI ( 0.07 Gy/min ; day 0 ) 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The conditioning regimen consisted of fludarabine 30 mg/m ( 2 ) / day ( days -5 , -4 , -3 ) and 2 Gy TBI ( 0.07 Gy/min ; day 0 ) .
	manualset3
144969	1	409273	5	NULL	NULL	0	NULL	conformation 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformation of the N-H bond in the structure of the title compound , C ( 8 ) H ( 7 ) BrClNO , is syn to the 2-chloro substituent in the aniline ring and anti to both the C = O and C-Br bonds in the side chain , similar to that observed in 2-chloro-N - ( 2-chloro-phen-yl ) acetamide .
	manualset3
144970	2	409273	5	NULL	NULL	0	NULL	N-H bond 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformation of the N-H bond in the structure of the title compound , C ( 8 ) H ( 7 ) BrClNO , is syn to the 2-chloro substituent in the aniline ring and anti to both the C = O and C-Br bonds in the side chain , similar to that observed in 2-chloro-N - ( 2-chloro-phen-yl ) acetamide .
	manualset3
144971	3	409273	5	NULL	NULL	0	NULL	structure 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformation of the N-H bond in the structure of the title compound , C ( 8 ) H ( 7 ) BrClNO , is syn to the 2-chloro substituent in the aniline ring and anti to both the C = O and C-Br bonds in the side chain , similar to that observed in 2-chloro-N - ( 2-chloro-phen-yl ) acetamide .
	manualset3
144972	4	409273	5	NULL	NULL	NULL	NULL	title compound , C ( 8 ) H ( 7 ) BrClNO	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The conformation of the N-H bond in the structure of the title compound , C ( 8 ) H ( 7 ) BrClNO , is syn to the 2-chloro substituent in the aniline ring and anti to both the C = O and C-Br bonds in the side chain , similar to that observed in 2-chloro-N - ( 2-chloro-phen-yl ) acetamide .
	manualset3
144973	5	409273	5	NULL	NULL	0	NULL	2-chloro substituent 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformation of the N-H bond in the structure of the title compound , C ( 8 ) H ( 7 ) BrClNO , is syn to the 2-chloro substituent in the aniline ring and anti to both the C = O and C-Br bonds in the side chain , similar to that observed in 2-chloro-N - ( 2-chloro-phen-yl ) acetamide .
	manualset3
144974	6	409273	5	NULL	NULL	0	NULL	aniline ring	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformation of the N-H bond in the structure of the title compound , C ( 8 ) H ( 7 ) BrClNO , is syn to the 2-chloro substituent in the aniline ring and anti to both the C = O and C-Br bonds in the side chain , similar to that observed in 2-chloro-N - ( 2-chloro-phen-yl ) acetamide .
	manualset3
144975	7	409273	5	NULL	NULL	0	NULL	 C = O bond	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformation of the N-H bond in the structure of the title compound , C ( 8 ) H ( 7 ) BrClNO , is syn to the 2-chloro substituent in the aniline ring and anti to both the C = O and C-Br bonds in the side chain , similar to that observed in 2-chloro-N - ( 2-chloro-phen-yl ) acetamide .
	manualset3
144976	8	409273	5	NULL	NULL	0	NULL	C-Br bond	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformation of the N-H bond in the structure of the title compound , C ( 8 ) H ( 7 ) BrClNO , is syn to the 2-chloro substituent in the aniline ring and anti to both the C = O and C-Br bonds in the side chain , similar to that observed in 2-chloro-N - ( 2-chloro-phen-yl ) acetamide .
	manualset3
144977	9	409273	5	NULL	NULL	0	NULL	side chain	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformation of the N-H bond in the structure of the title compound , C ( 8 ) H ( 7 ) BrClNO , is syn to the 2-chloro substituent in the aniline ring and anti to both the C = O and C-Br bonds in the side chain , similar to that observed in 2-chloro-N - ( 2-chloro-phen-yl ) acetamide .
	manualset3
144978	10	409273	5	NULL	NULL	0	NULL	2-chloro-N - ( 2-chloro-phen-yl ) acetamide	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformation of the N-H bond in the structure of the title compound , C ( 8 ) H ( 7 ) BrClNO , is syn to the 2-chloro substituent in the aniline ring and anti to both the C = O and C-Br bonds in the side chain , similar to that observed in 2-chloro-N - ( 2-chloro-phen-yl ) acetamide .
	manualset3
144979	1	409274	5	NULL	NULL	0	NULL	conformation 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformation of the double-stranded , mixed ribodeoxyribo polynucleotide , poly ( rG-dC ) .
	manualset3
144980	2	409274	5	NULL	NULL	0	NULL	double-stranded , mixed ribodeoxyribo polynucleotide , poly ( rG-dC )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformation of the double-stranded , mixed ribodeoxyribo polynucleotide , poly ( rG-dC ) .
	manualset3
144981	1	409275	5	NULL	NULL	0	NULL	conformational analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformational analysis of ( sequence : see text ) the disulphide cyclopeptide-related cyclolinopeptide A , has been carried out by solid state methods using x-ray diffraction techniques , in solution by nmr , CD , ir spectroscopies , and by molecular dynamics ( MD ) analysis .
	manualset3
144982	2	409275	5	NULL	NULL	0	NULL	sequence 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformational analysis of ( sequence : see text ) the disulphide cyclopeptide-related cyclolinopeptide A , has been carried out by solid state methods using x-ray diffraction techniques , in solution by nmr , CD , ir spectroscopies , and by molecular dynamics ( MD ) analysis .
	manualset3
144983	3	409275	5	NULL	NULL	0	NULL	disulphide cyclopeptide-related cyclolinopeptide A	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformational analysis of ( sequence : see text ) the disulphide cyclopeptide-related cyclolinopeptide A , has been carried out by solid state methods using x-ray diffraction techniques , in solution by nmr , CD , ir spectroscopies , and by molecular dynamics ( MD ) analysis .
	manualset3
144984	4	409275	5	NULL	NULL	0	NULL	solid state methods 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformational analysis of ( sequence : see text ) the disulphide cyclopeptide-related cyclolinopeptide A , has been carried out by solid state methods using x-ray diffraction techniques , in solution by nmr , CD , ir spectroscopies , and by molecular dynamics ( MD ) analysis .
	manualset3
144985	5	409275	5	NULL	NULL	0	NULL	x-ray diffraction techniques 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformational analysis of ( sequence : see text ) the disulphide cyclopeptide-related cyclolinopeptide A , has been carried out by solid state methods using x-ray diffraction techniques , in solution by nmr , CD , ir spectroscopies , and by molecular dynamics ( MD ) analysis .
	manualset3
144986	6	409275	5	NULL	NULL	0	NULL	solution 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformational analysis of ( sequence : see text ) the disulphide cyclopeptide-related cyclolinopeptide A , has been carried out by solid state methods using x-ray diffraction techniques , in solution by nmr , CD , ir spectroscopies , and by molecular dynamics ( MD ) analysis .
	manualset3
144987	7	409275	5	NULL	NULL	0	NULL	nmr 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformational analysis of ( sequence : see text ) the disulphide cyclopeptide-related cyclolinopeptide A , has been carried out by solid state methods using x-ray diffraction techniques , in solution by nmr , CD , ir spectroscopies , and by molecular dynamics ( MD ) analysis .
	manualset3
144988	8	409275	5	NULL	NULL	0	NULL	CD 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformational analysis of ( sequence : see text ) the disulphide cyclopeptide-related cyclolinopeptide A , has been carried out by solid state methods using x-ray diffraction techniques , in solution by nmr , CD , ir spectroscopies , and by molecular dynamics ( MD ) analysis .
	manualset3
144989	9	409275	5	NULL	NULL	0	NULL	ir spectroscopies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformational analysis of ( sequence : see text ) the disulphide cyclopeptide-related cyclolinopeptide A , has been carried out by solid state methods using x-ray diffraction techniques , in solution by nmr , CD , ir spectroscopies , and by molecular dynamics ( MD ) analysis .
	manualset3
144990	10	409275	5	NULL	NULL	0	NULL	molecular dynamics ( MD ) analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformational analysis of ( sequence : see text ) the disulphide cyclopeptide-related cyclolinopeptide A , has been carried out by solid state methods using x-ray diffraction techniques , in solution by nmr , CD , ir spectroscopies , and by molecular dynamics ( MD ) analysis .
	manualset3
144991	1	409276	5	NULL	NULL	0	NULL	significant positive correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant positive correlation between Token Test scores and paragraph scores was observed for high-level aphasic subjects ; the correlation between these measures was low and nonsignificant for low-level aphasic subjects .
	manualset3
144992	2	409276	5	NULL	NULL	0	NULL	Token Test scores	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant positive correlation between Token Test scores and paragraph scores was observed for high-level aphasic subjects ; the correlation between these measures was low and nonsignificant for low-level aphasic subjects .
	manualset3
144993	3	409276	5	NULL	NULL	0	NULL	paragraph scores	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant positive correlation between Token Test scores and paragraph scores was observed for high-level aphasic subjects ; the correlation between these measures was low and nonsignificant for low-level aphasic subjects .
	manualset3
144994	4	409276	5	NULL	NULL	0	NULL	high-level aphasic subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant positive correlation between Token Test scores and paragraph scores was observed for high-level aphasic subjects ; the correlation between these measures was low and nonsignificant for low-level aphasic subjects .
	manualset3
144995	5	409276	5	NULL	NULL	0	NULL	correlation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant positive correlation between Token Test scores and paragraph scores was observed for high-level aphasic subjects ; the correlation between these measures was low and nonsignificant for low-level aphasic subjects .
	manualset3
144996	6	409276	5	NULL	NULL	0	NULL	measures 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant positive correlation between Token Test scores and paragraph scores was observed for high-level aphasic subjects ; the correlation between these measures was low and nonsignificant for low-level aphasic subjects .
	manualset3
144997	7	409276	5	NULL	NULL	0	NULL	low-level aphasic subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant positive correlation between Token Test scores and paragraph scores was observed for high-level aphasic subjects ; the correlation between these measures was low and nonsignificant for low-level aphasic subjects .
	manualset3
144998	1	409277	5	NULL	NULL	0	NULL	conformational analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformational and quantum analyses of dental adhesive carboxylic acid and carboxylic acid anhydride monomers were preformed .
	manualset3
144999	2	409277	5	NULL	NULL	0	NULL	quantum analyses 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformational and quantum analyses of dental adhesive carboxylic acid and carboxylic acid anhydride monomers were preformed .
	manualset3
145000	3	409277	5	NULL	NULL	0	NULL	dental adhesive carboxylic acid	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformational and quantum analyses of dental adhesive carboxylic acid and carboxylic acid anhydride monomers were preformed .
	manualset3
145001	4	409277	5	NULL	NULL	0	NULL	carboxylic acid anhydride monomers	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformational and quantum analyses of dental adhesive carboxylic acid and carboxylic acid anhydride monomers were preformed .
	manualset3
145002	1	409278	5	NULL	NULL	0	NULL	conformations 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformations of two backbone-cyclized substance P analogs were derived from homo - and heteronuclear NMR measurements and molecular dynamics simulations carried out in DMSO .
	manualset3
145003	2	409278	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformations of two backbone-cyclized substance P analogs were derived from homo - and heteronuclear NMR measurements and molecular dynamics simulations carried out in DMSO .
	manualset3
145004	3	409278	5	NULL	NULL	0	NULL	backbone-cyclized substance P analogs	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformations of two backbone-cyclized substance P analogs were derived from homo - and heteronuclear NMR measurements and molecular dynamics simulations carried out in DMSO .
	manualset3
145005	4	409278	5	NULL	NULL	0	NULL	homonuclear NMR measurements	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformations of two backbone-cyclized substance P analogs were derived from homo - and heteronuclear NMR measurements and molecular dynamics simulations carried out in DMSO .
	manualset3
145006	5	409278	5	NULL	NULL	0	NULL	heteronuclear NMR measurements	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformations of two backbone-cyclized substance P analogs were derived from homo - and heteronuclear NMR measurements and molecular dynamics simulations carried out in DMSO .
	manualset3
145007	6	409278	5	NULL	NULL	0	NULL	molecular dynamics simulations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformations of two backbone-cyclized substance P analogs were derived from homo - and heteronuclear NMR measurements and molecular dynamics simulations carried out in DMSO .
	manualset3
145008	7	409278	5	NULL	NULL	0	NULL	DMSO 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The conformations of two backbone-cyclized substance P analogs were derived from homo - and heteronuclear NMR measurements and molecular dynamics simulations carried out in DMSO .
	manualset3
145009	1	409279	5	NULL	NULL	0	NULL	congenital fistula	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The congenital fistula of the 4th branchial pouch is rare .
	manualset3
145010	2	409279	5	NULL	NULL	0	NULL	branchial pouch	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The congenital fistula of the 4th branchial pouch is rare .
	manualset3
145011	1	409280	5	NULL	NULL	0	NULL	connective tissue 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The connective tissue was newly developed between the skin basement membrane and thick collagen lamella in the body but not in the tail .
	manualset3
145012	2	409280	5	NULL	NULL	0	NULL	skin basement membrane	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The connective tissue was newly developed between the skin basement membrane and thick collagen lamella in the body but not in the tail .
	manualset3
145013	3	409280	5	NULL	NULL	0	NULL	thick collagen lamella	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The connective tissue was newly developed between the skin basement membrane and thick collagen lamella in the body but not in the tail .
	manualset3
145014	4	409280	5	NULL	NULL	0	NULL	body 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The connective tissue was newly developed between the skin basement membrane and thick collagen lamella in the body but not in the tail .
	manualset3
145015	5	409280	5	NULL	NULL	0	NULL	tail 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The connective tissue was newly developed between the skin basement membrane and thick collagen lamella in the body but not in the tail .
	manualset3
145016	1	409281	5	NULL	NULL	0	NULL	consensus clinical opinion 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The consensus clinical opinion was used as the gold standard to differentiate between preparatory grief and depression .
	manualset3
145017	2	409281	5	NULL	NULL	0	NULL	gold standard	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The consensus clinical opinion was used as the gold standard to differentiate between preparatory grief and depression .
	manualset3
145018	3	409281	5	NULL	NULL	0	NULL	preparatory grief 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The consensus clinical opinion was used as the gold standard to differentiate between preparatory grief and depression .
	manualset3
145019	4	409281	5	NULL	NULL	0	NULL	depression 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The consensus clinical opinion was used as the gold standard to differentiate between preparatory grief and depression .
	manualset3
145020	1	409282	5	NULL	NULL	0	NULL	consequences 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The consequences of hypovolemia include reduction in circulating blood volume , lower venous return and , in profound cases , arterial hypotension .
	manualset3
145021	2	409282	5	NULL	NULL	0	NULL	hypovolemia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The consequences of hypovolemia include reduction in circulating blood volume , lower venous return and , in profound cases , arterial hypotension .
	manualset3
145022	3	409282	5	NULL	NULL	NULL	NULL	reduction 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The consequences of hypovolemia include reduction in circulating blood volume , lower venous return and , in profound cases , arterial hypotension .
	manualset3
145023	4	409282	5	NULL	NULL	0	NULL	circulating blood volume	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The consequences of hypovolemia include reduction in circulating blood volume , lower venous return and , in profound cases , arterial hypotension .
	manualset3
145024	5	409282	5	NULL	NULL	0	NULL	lower venous return	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The consequences of hypovolemia include reduction in circulating blood volume , lower venous return and , in profound cases , arterial hypotension .
	manualset3
145025	6	409282	5	NULL	NULL	0	NULL	profound cases	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The consequences of hypovolemia include reduction in circulating blood volume , lower venous return and , in profound cases , arterial hypotension .
	manualset3
145026	7	409282	5	NULL	NULL	0	NULL	arterial hypotension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The consequences of hypovolemia include reduction in circulating blood volume , lower venous return and , in profound cases , arterial hypotension .
	manualset3
145027	1	409283	5	NULL	NULL	0	NULL	constitutive association	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The constitutive association of U1 small nuclear ribonucleoprotein ( snRNP ) with the transcription machinery might play a role in coupling transcription with pre-mRNA maturation .
	manualset3
145028	2	409283	5	NULL	NULL	0	NULL	U1 small nuclear ribonucleoprotein ( snRNP ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The constitutive association of U1 small nuclear ribonucleoprotein ( snRNP ) with the transcription machinery might play a role in coupling transcription with pre-mRNA maturation .
	manualset3
145029	3	409283	5	NULL	NULL	0	NULL	transcription machinery	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The constitutive association of U1 small nuclear ribonucleoprotein ( snRNP ) with the transcription machinery might play a role in coupling transcription with pre-mRNA maturation .
	manualset3
145030	4	409283	5	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The constitutive association of U1 small nuclear ribonucleoprotein ( snRNP ) with the transcription machinery might play a role in coupling transcription with pre-mRNA maturation .
	manualset3
145031	5	409283	5	NULL	NULL	0	NULL	transcription 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The constitutive association of U1 small nuclear ribonucleoprotein ( snRNP ) with the transcription machinery might play a role in coupling transcription with pre-mRNA maturation .
	manualset3
145032	6	409283	5	NULL	NULL	0	NULL	pre-mRNA maturation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The constitutive association of U1 small nuclear ribonucleoprotein ( snRNP ) with the transcription machinery might play a role in coupling transcription with pre-mRNA maturation .
	manualset3
145033	1	409284	5	NULL	NULL	0	NULL	consultants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The consultants also agree that certain studies should be obtained prior to a biopsy .
	manualset3
145034	2	409284	5	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The consultants also agree that certain studies should be obtained prior to a biopsy .
	manualset3
145035	3	409284	5	NULL	NULL	0	NULL	biopsy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The consultants also agree that certain studies should be obtained prior to a biopsy .
	manualset3
145036	1	409285	5	NULL	NULL	0	NULL	significant positive relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant positive relationship was found between adipose tissue UDP-N-acetylglucosamine and BMI ( Spearman correlation = 0.576 ; P = 0.0007 ) and between UDP-N-acetylglucosamine and serum leptin ( Spearman correlation = 0.4650 ; P = 0.0145 ) .
	manualset3
145037	2	409285	5	NULL	NULL	0	NULL	adipose tissue UDP-N-acetylglucosamine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant positive relationship was found between adipose tissue UDP-N-acetylglucosamine and BMI ( Spearman correlation = 0.576 ; P = 0.0007 ) and between UDP-N-acetylglucosamine and serum leptin ( Spearman correlation = 0.4650 ; P = 0.0145 ) .
	manualset3
145038	3	409285	5	NULL	NULL	0	NULL	BMI 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant positive relationship was found between adipose tissue UDP-N-acetylglucosamine and BMI ( Spearman correlation = 0.576 ; P = 0.0007 ) and between UDP-N-acetylglucosamine and serum leptin ( Spearman correlation = 0.4650 ; P = 0.0145 ) .
	manualset3
145039	4	409285	5	NULL	NULL	0	NULL	Spearman correlation = 0.576	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant positive relationship was found between adipose tissue UDP-N-acetylglucosamine and BMI ( Spearman correlation = 0.576 ; P = 0.0007 ) and between UDP-N-acetylglucosamine and serum leptin ( Spearman correlation = 0.4650 ; P = 0.0145 ) .
	manualset3
145040	5	409285	5	NULL	NULL	0	NULL	P = 0.0007	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant positive relationship was found between adipose tissue UDP-N-acetylglucosamine and BMI ( Spearman correlation = 0.576 ; P = 0.0007 ) and between UDP-N-acetylglucosamine and serum leptin ( Spearman correlation = 0.4650 ; P = 0.0145 ) .
	manualset3
145041	6	409285	5	NULL	NULL	0	NULL	UDP-N-acetylglucosamine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant positive relationship was found between adipose tissue UDP-N-acetylglucosamine and BMI ( Spearman correlation = 0.576 ; P = 0.0007 ) and between UDP-N-acetylglucosamine and serum leptin ( Spearman correlation = 0.4650 ; P = 0.0145 ) .
	manualset3
145042	7	409285	5	NULL	NULL	0	NULL	serum leptin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant positive relationship was found between adipose tissue UDP-N-acetylglucosamine and BMI ( Spearman correlation = 0.576 ; P = 0.0007 ) and between UDP-N-acetylglucosamine and serum leptin ( Spearman correlation = 0.4650 ; P = 0.0145 ) .
	manualset3
145043	8	409285	5	NULL	NULL	0	NULL	Spearman correlation = 0.4650	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant positive relationship was found between adipose tissue UDP-N-acetylglucosamine and BMI ( Spearman correlation = 0.576 ; P = 0.0007 ) and between UDP-N-acetylglucosamine and serum leptin ( Spearman correlation = 0.4650 ; P = 0.0145 ) .
	manualset3
145044	9	409285	5	NULL	NULL	0	NULL	P = 0.0145 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant positive relationship was found between adipose tissue UDP-N-acetylglucosamine and BMI ( Spearman correlation = 0.576 ; P = 0.0007 ) and between UDP-N-acetylglucosamine and serum leptin ( Spearman correlation = 0.4650 ; P = 0.0145 ) .
	manualset3
145045	1	409286	5	NULL	NULL	0	NULL	contemporary American abortion controversy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The contemporary American abortion controversy : stages in the argument .
	manualset3
145046	2	409286	5	NULL	NULL	0	NULL	stages 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The contemporary American abortion controversy : stages in the argument .
	manualset3
145047	3	409286	5	NULL	NULL	0	NULL	argument 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The contemporary American abortion controversy : stages in the argument .
	manualset3
145048	1	409287	5	NULL	NULL	0	NULL	content 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The content and format is similar to that of non-magnetic subperiodic groups and space groups given in International Tables for Crystallography .
	manualset3
145049	2	409287	5	NULL	NULL	0	NULL	format 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The content and format is similar to that of non-magnetic subperiodic groups and space groups given in International Tables for Crystallography .
	manualset3
145050	3	409287	5	NULL	NULL	0	NULL	non-magnetic subperiodic groups	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The content and format is similar to that of non-magnetic subperiodic groups and space groups given in International Tables for Crystallography .
	manualset3
145051	4	409287	5	NULL	NULL	0	NULL	space groups 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The content and format is similar to that of non-magnetic subperiodic groups and space groups given in International Tables for Crystallography .
	manualset3
145052	5	409287	5	NULL	NULL	0	NULL	International Tables for Crystallography	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The content and format is similar to that of non-magnetic subperiodic groups and space groups given in International Tables for Crystallography .
	manualset3
145053	1	409288	5	NULL	NULL	NULL	NULL	content of polysomes per unit liver tissue	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The content of polysomes per unit liver tissue from 7 groups of fed mice aged 10 -- 35 months showed an age-related increase of subunits and monomers ( +54 % ) and dimers-to-pentamers ( +76 % ) in membrane-bound polyribosomes .
	manualset3
145054	2	409288	5	NULL	NULL	0	NULL	7 groups	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The content of polysomes per unit liver tissue from 7 groups of fed mice aged 10 -- 35 months showed an age-related increase of subunits and monomers ( +54 % ) and dimers-to-pentamers ( +76 % ) in membrane-bound polyribosomes .
	manualset3
145055	3	409288	5	NULL	NULL	0	NULL	fed mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The content of polysomes per unit liver tissue from 7 groups of fed mice aged 10 -- 35 months showed an age-related increase of subunits and monomers ( +54 % ) and dimers-to-pentamers ( +76 % ) in membrane-bound polyribosomes .
	manualset3
145056	4	409288	5	NULL	NULL	0	NULL	10 -- 35 months 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The content of polysomes per unit liver tissue from 7 groups of fed mice aged 10 -- 35 months showed an age-related increase of subunits and monomers ( +54 % ) and dimers-to-pentamers ( +76 % ) in membrane-bound polyribosomes .
	manualset3
145057	5	409288	5	NULL	NULL	0	NULL	age-related increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The content of polysomes per unit liver tissue from 7 groups of fed mice aged 10 -- 35 months showed an age-related increase of subunits and monomers ( +54 % ) and dimers-to-pentamers ( +76 % ) in membrane-bound polyribosomes .
	manualset3
145058	6	409288	5	NULL	NULL	0	NULL	subunits 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The content of polysomes per unit liver tissue from 7 groups of fed mice aged 10 -- 35 months showed an age-related increase of subunits and monomers ( +54 % ) and dimers-to-pentamers ( +76 % ) in membrane-bound polyribosomes .
	manualset3
145059	7	409288	5	NULL	NULL	0	NULL	monomers 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The content of polysomes per unit liver tissue from 7 groups of fed mice aged 10 -- 35 months showed an age-related increase of subunits and monomers ( +54 % ) and dimers-to-pentamers ( +76 % ) in membrane-bound polyribosomes .
	manualset3
145060	8	409288	5	NULL	NULL	0	NULL	+54 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The content of polysomes per unit liver tissue from 7 groups of fed mice aged 10 -- 35 months showed an age-related increase of subunits and monomers ( +54 % ) and dimers-to-pentamers ( +76 % ) in membrane-bound polyribosomes .
	manualset3
145061	9	409288	5	NULL	NULL	0	NULL	dimers	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The content of polysomes per unit liver tissue from 7 groups of fed mice aged 10 -- 35 months showed an age-related increase of subunits and monomers ( +54 % ) and dimers-to-pentamers ( +76 % ) in membrane-bound polyribosomes .
	manualset3
145062	10	409288	5	NULL	NULL	0	NULL	pentamers 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The content of polysomes per unit liver tissue from 7 groups of fed mice aged 10 -- 35 months showed an age-related increase of subunits and monomers ( +54 % ) and dimers-to-pentamers ( +76 % ) in membrane-bound polyribosomes .
	manualset3
145063	11	409288	5	NULL	NULL	0	NULL	+76 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The content of polysomes per unit liver tissue from 7 groups of fed mice aged 10 -- 35 months showed an age-related increase of subunits and monomers ( +54 % ) and dimers-to-pentamers ( +76 % ) in membrane-bound polyribosomes .
	manualset3
145064	12	409288	5	NULL	NULL	0	NULL	membrane-bound polyribosomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The content of polysomes per unit liver tissue from 7 groups of fed mice aged 10 -- 35 months showed an age-related increase of subunits and monomers ( +54 % ) and dimers-to-pentamers ( +76 % ) in membrane-bound polyribosomes .
	manualset3
145065	1	409289	5	NULL	NULL	NULL	NULL	contents 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The contents of V , Cr , Co , Ni , Cu , Ga , Rb , Cd , Ba , and Pb in the soft tissue of blue mussel ( Mytilus edulis ) were determined by a high resolution inductively coupled plasma mass spectrometry ( HR-ICPMS ) method .
	manualset3
145066	2	409289	5	NULL	NULL	0	NULL	 V	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The contents of V , Cr , Co , Ni , Cu , Ga , Rb , Cd , Ba , and Pb in the soft tissue of blue mussel ( Mytilus edulis ) were determined by a high resolution inductively coupled plasma mass spectrometry ( HR-ICPMS ) method .
	manualset3
145067	3	409289	5	NULL	NULL	0	NULL	Cr 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The contents of V , Cr , Co , Ni , Cu , Ga , Rb , Cd , Ba , and Pb in the soft tissue of blue mussel ( Mytilus edulis ) were determined by a high resolution inductively coupled plasma mass spectrometry ( HR-ICPMS ) method .
	manualset3
145068	4	409289	5	NULL	NULL	0	NULL	Co 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The contents of V , Cr , Co , Ni , Cu , Ga , Rb , Cd , Ba , and Pb in the soft tissue of blue mussel ( Mytilus edulis ) were determined by a high resolution inductively coupled plasma mass spectrometry ( HR-ICPMS ) method .
	manualset3
145069	5	409289	5	NULL	NULL	0	NULL	Ni 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The contents of V , Cr , Co , Ni , Cu , Ga , Rb , Cd , Ba , and Pb in the soft tissue of blue mussel ( Mytilus edulis ) were determined by a high resolution inductively coupled plasma mass spectrometry ( HR-ICPMS ) method .
	manualset3
145070	6	409289	5	NULL	NULL	0	NULL	Cu 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The contents of V , Cr , Co , Ni , Cu , Ga , Rb , Cd , Ba , and Pb in the soft tissue of blue mussel ( Mytilus edulis ) were determined by a high resolution inductively coupled plasma mass spectrometry ( HR-ICPMS ) method .
	manualset3
145071	7	409289	5	NULL	NULL	0	NULL	Ga 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The contents of V , Cr , Co , Ni , Cu , Ga , Rb , Cd , Ba , and Pb in the soft tissue of blue mussel ( Mytilus edulis ) were determined by a high resolution inductively coupled plasma mass spectrometry ( HR-ICPMS ) method .
	manualset3
145072	8	409289	5	NULL	NULL	0	NULL	Rb 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The contents of V , Cr , Co , Ni , Cu , Ga , Rb , Cd , Ba , and Pb in the soft tissue of blue mussel ( Mytilus edulis ) were determined by a high resolution inductively coupled plasma mass spectrometry ( HR-ICPMS ) method .
	manualset3
145073	9	409289	5	NULL	NULL	0	NULL	Cd 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The contents of V , Cr , Co , Ni , Cu , Ga , Rb , Cd , Ba , and Pb in the soft tissue of blue mussel ( Mytilus edulis ) were determined by a high resolution inductively coupled plasma mass spectrometry ( HR-ICPMS ) method .
	manualset3
145074	10	409289	5	NULL	NULL	0	NULL	Ba 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The contents of V , Cr , Co , Ni , Cu , Ga , Rb , Cd , Ba , and Pb in the soft tissue of blue mussel ( Mytilus edulis ) were determined by a high resolution inductively coupled plasma mass spectrometry ( HR-ICPMS ) method .
	manualset3
145075	11	409289	5	NULL	NULL	0	NULL	Pb 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The contents of V , Cr , Co , Ni , Cu , Ga , Rb , Cd , Ba , and Pb in the soft tissue of blue mussel ( Mytilus edulis ) were determined by a high resolution inductively coupled plasma mass spectrometry ( HR-ICPMS ) method .
	manualset3
145076	12	409289	5	NULL	NULL	0	NULL	soft tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The contents of V , Cr , Co , Ni , Cu , Ga , Rb , Cd , Ba , and Pb in the soft tissue of blue mussel ( Mytilus edulis ) were determined by a high resolution inductively coupled plasma mass spectrometry ( HR-ICPMS ) method .
	manualset3
145077	13	409289	5	NULL	NULL	0	NULL	blue mussel ( Mytilus edulis )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The contents of V , Cr , Co , Ni , Cu , Ga , Rb , Cd , Ba , and Pb in the soft tissue of blue mussel ( Mytilus edulis ) were determined by a high resolution inductively coupled plasma mass spectrometry ( HR-ICPMS ) method .
	manualset3
145078	14	409289	5	NULL	NULL	0	NULL	high resolution inductively coupled plasma mass spectrometry ( HR-ICPMS ) method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The contents of V , Cr , Co , Ni , Cu , Ga , Rb , Cd , Ba , and Pb in the soft tissue of blue mussel ( Mytilus edulis ) were determined by a high resolution inductively coupled plasma mass spectrometry ( HR-ICPMS ) method .
	manualset3
145079	1	409290	5	NULL	NULL	0	NULL	contents 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The contents of both total collagen and the cross-linked type I and type III collagens in the malignant samples were only about 20 % of those in the benign tumors .
	manualset3
145080	2	409290	5	NULL	NULL	0	NULL	total collagen	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The contents of both total collagen and the cross-linked type I and type III collagens in the malignant samples were only about 20 % of those in the benign tumors .
	manualset3
145081	3	409290	5	NULL	NULL	0	NULL	cross-linked type I collagen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The contents of both total collagen and the cross-linked type I and type III collagens in the malignant samples were only about 20 % of those in the benign tumors .
	manualset3
145082	4	409290	5	NULL	NULL	0	NULL	cross-linked type III collagen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The contents of both total collagen and the cross-linked type I and type III collagens in the malignant samples were only about 20 % of those in the benign tumors .
	manualset3
145083	5	409290	5	NULL	NULL	0	NULL	malignant samples	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The contents of both total collagen and the cross-linked type I and type III collagens in the malignant samples were only about 20 % of those in the benign tumors .
	manualset3
145084	6	409290	5	NULL	NULL	0	NULL	20 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The contents of both total collagen and the cross-linked type I and type III collagens in the malignant samples were only about 20 % of those in the benign tumors .
	manualset3
145085	7	409290	5	NULL	NULL	0	NULL	benign tumors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The contents of both total collagen and the cross-linked type I and type III collagens in the malignant samples were only about 20 % of those in the benign tumors .
	manualset3
145086	1	409291	5	NULL	NULL	0	NULL	contents 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The contents of minerals were determined by flame AAS .
	manualset3
145087	2	409291	5	NULL	NULL	0	NULL	minerals 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The contents of minerals were determined by flame AAS .
	manualset3
145088	3	409291	5	NULL	NULL	0	NULL	flame AAS	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The contents of minerals were determined by flame AAS .
	manualset3
145089	1	409292	5	NULL	NULL	0	NULL	laboratory scale Kaldnes	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The continuously operated laboratory scale Kaldnes moving bed biofilm reactor ( MBBR ) was used for thermophilic ( 55 degrees C ) aerobic treatment of TMP whitewater .
	manualset3
145090	2	409292	5	NULL	NULL	0	NULL	moving bed biofilm reactor ( MBBR ) 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The continuously operated laboratory scale Kaldnes moving bed biofilm reactor ( MBBR ) was used for thermophilic ( 55 degrees C ) aerobic treatment of TMP whitewater .
	manualset3
145091	3	409292	5	NULL	NULL	0	NULL	thermophilic aerobic treatment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The continuously operated laboratory scale Kaldnes moving bed biofilm reactor ( MBBR ) was used for thermophilic ( 55 degrees C ) aerobic treatment of TMP whitewater .
	manualset3
145092	4	409292	5	NULL	NULL	0	NULL	55 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The continuously operated laboratory scale Kaldnes moving bed biofilm reactor ( MBBR ) was used for thermophilic ( 55 degrees C ) aerobic treatment of TMP whitewater .
	manualset3
145093	5	409292	5	NULL	NULL	0	NULL	TMP whitewater	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The continuously operated laboratory scale Kaldnes moving bed biofilm reactor ( MBBR ) was used for thermophilic ( 55 degrees C ) aerobic treatment of TMP whitewater .
	manualset3
145094	1	409293	5	NULL	NULL	0	NULL	contraction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The contraction induced by EFS was inhibited by nitric oxide , but potentiated by the nitric oxide-synthase inhibitor , L-NAME .
	manualset3
145095	2	409293	5	NULL	NULL	0	NULL	EFS 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The contraction induced by EFS was inhibited by nitric oxide , but potentiated by the nitric oxide-synthase inhibitor , L-NAME .
	manualset3
145096	3	409293	5	NULL	NULL	0	NULL	nitric oxide	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The contraction induced by EFS was inhibited by nitric oxide , but potentiated by the nitric oxide-synthase inhibitor , L-NAME .
	manualset3
145097	4	409293	5	NULL	NULL	0	NULL	nitric oxide-synthase inhibitor , L-NAME	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The contraction induced by EFS was inhibited by nitric oxide , but potentiated by the nitric oxide-synthase inhibitor , L-NAME .
	manualset3
145098	1	409294	5	NULL	NULL	0	NULL	contractures 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The contractures were produced almost exclusively by a loss in the extension range of motion .
	manualset3
145099	2	409294	5	NULL	NULL	0	NULL	loss 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The contractures were produced almost exclusively by a loss in the extension range of motion .
	manualset3
145100	3	409294	5	NULL	NULL	0	NULL	extension range of motion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The contractures were produced almost exclusively by a loss in the extension range of motion .
	manualset3
145101	1	409295	5	NULL	NULL	0	NULL	contribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The contribution of mitochondrial calcium ion exchange to relaxation of tension in cardiac muscle .
	manualset3
145102	2	409295	5	NULL	NULL	0	NULL	mitochondrial calcium ion exchange	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The contribution of mitochondrial calcium ion exchange to relaxation of tension in cardiac muscle .
	manualset3
145103	3	409295	5	NULL	NULL	0	NULL	relaxation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The contribution of mitochondrial calcium ion exchange to relaxation of tension in cardiac muscle .
	manualset3
145104	4	409295	5	NULL	NULL	0	NULL	tension 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The contribution of mitochondrial calcium ion exchange to relaxation of tension in cardiac muscle .
	manualset3
145105	5	409295	5	NULL	NULL	0	NULL	cardiac muscle	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The contribution of mitochondrial calcium ion exchange to relaxation of tension in cardiac muscle .
	manualset3
145106	1	409296	5	NULL	NULL	0	NULL	contribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The contribution of regenerated thermoluminescence to low doses is studied for the case of CaF2-Dy ( TLD-200 ) .
	manualset3
145107	2	409296	5	NULL	NULL	0	NULL	regenerated thermoluminescence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The contribution of regenerated thermoluminescence to low doses is studied for the case of CaF2-Dy ( TLD-200 ) .
	manualset3
145108	3	409296	5	NULL	NULL	0	NULL	low doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The contribution of regenerated thermoluminescence to low doses is studied for the case of CaF2-Dy ( TLD-200 ) .
	manualset3
145109	4	409296	5	NULL	NULL	0	NULL	case 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The contribution of regenerated thermoluminescence to low doses is studied for the case of CaF2-Dy ( TLD-200 ) .
	manualset3
145110	5	409296	5	NULL	NULL	0	NULL	CaF2-Dy ( TLD-200 )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The contribution of regenerated thermoluminescence to low doses is studied for the case of CaF2-Dy ( TLD-200 ) .
	manualset3
145111	1	409297	5	NULL	NULL	0	NULL	control 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The control and coordination of eukaryotic gene expression rely on transcriptional and post-transcriptional regulatory networks .
	manualset3
145112	2	409297	5	NULL	NULL	0	NULL	coordination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The control and coordination of eukaryotic gene expression rely on transcriptional and post-transcriptional regulatory networks .
	manualset3
145113	3	409297	5	NULL	NULL	0	NULL	eukaryotic gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The control and coordination of eukaryotic gene expression rely on transcriptional and post-transcriptional regulatory networks .
	manualset3
145114	4	409297	5	NULL	NULL	0	NULL	transcriptional regulatory networks	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The control and coordination of eukaryotic gene expression rely on transcriptional and post-transcriptional regulatory networks .
	manualset3
145115	5	409297	5	NULL	NULL	0	NULL	post-transcriptional regulatory networks	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The control and coordination of eukaryotic gene expression rely on transcriptional and post-transcriptional regulatory networks .
	manualset3
145116	1	409298	5	NULL	NULL	0	NULL	significant relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant relationship was found between positivity and abortion in ewes .
	manualset3
145117	2	409298	5	NULL	NULL	0	NULL	positivity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant relationship was found between positivity and abortion in ewes .
	manualset3
145118	3	409298	5	NULL	NULL	0	NULL	abortion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant relationship was found between positivity and abortion in ewes .
	manualset3
145119	4	409298	5	NULL	NULL	0	NULL	ewes 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant relationship was found between positivity and abortion in ewes .
	manualset3
145120	1	409299	5	NULL	NULL	0	NULL	control 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The control of infection through hygiene has a long erratic history .
	manualset3
145121	2	409299	5	NULL	NULL	0	NULL	infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The control of infection through hygiene has a long erratic history .
	manualset3
145122	3	409299	5	NULL	NULL	0	NULL	hygiene 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The control of infection through hygiene has a long erratic history .
	manualset3
145123	4	409299	5	NULL	NULL	0	NULL	erratic history	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The control of infection through hygiene has a long erratic history .
	manualset3
145124	1	409300	5	NULL	NULL	0	NULL	control 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The control of lymphoid leukosis in a flock White Plymouth Rock chickens .
	manualset3
145125	2	409300	5	NULL	NULL	0	NULL	lymphoid leukosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The control of lymphoid leukosis in a flock White Plymouth Rock chickens .
	manualset3
145126	3	409300	5	NULL	NULL	0	NULL	flock White Plymouth Rock chickens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The control of lymphoid leukosis in a flock White Plymouth Rock chickens .
	manualset3
145127	1	409301	5	NULL	NULL	0	NULL	controllable range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The controllable range of heating pattern was about 70 % of the distance from the center of the agar phantom in the direction of depth .
	manualset3
145128	2	409301	5	NULL	NULL	0	NULL	heating pattern	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The controllable range of heating pattern was about 70 % of the distance from the center of the agar phantom in the direction of depth .
	manualset3
145129	3	409301	5	NULL	NULL	0	NULL	70 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The controllable range of heating pattern was about 70 % of the distance from the center of the agar phantom in the direction of depth .
	manualset3
145130	4	409301	5	NULL	NULL	0	NULL	distance 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The controllable range of heating pattern was about 70 % of the distance from the center of the agar phantom in the direction of depth .
	manualset3
145131	5	409301	5	NULL	NULL	0	NULL	center 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The controllable range of heating pattern was about 70 % of the distance from the center of the agar phantom in the direction of depth .
	manualset3
145132	6	409301	5	NULL	NULL	0	NULL	agar phantom	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The controllable range of heating pattern was about 70 % of the distance from the center of the agar phantom in the direction of depth .
	manualset3
145133	7	409301	5	NULL	NULL	0	NULL	direction 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The controllable range of heating pattern was about 70 % of the distance from the center of the agar phantom in the direction of depth .
	manualset3
145134	8	409301	5	NULL	NULL	0	NULL	depth 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The controllable range of heating pattern was about 70 % of the distance from the center of the agar phantom in the direction of depth .
	manualset3
145135	1	409302	5	NULL	NULL	0	NULL	conventional method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The conventional method of assessing the platelet response to hypotonic stress ( HSR ) was adapted to allow microtitre plate technology to be used .
	manualset3
145136	2	409302	5	NULL	NULL	0	NULL	platelet response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The conventional method of assessing the platelet response to hypotonic stress ( HSR ) was adapted to allow microtitre plate technology to be used .
	manualset3
145137	3	409302	5	NULL	NULL	0	NULL	hypotonic stress ( HSR )	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The conventional method of assessing the platelet response to hypotonic stress ( HSR ) was adapted to allow microtitre plate technology to be used .
	manualset3
145138	4	409302	5	NULL	NULL	0	NULL	microtitre plate technology 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The conventional method of assessing the platelet response to hypotonic stress ( HSR ) was adapted to allow microtitre plate technology to be used .
	manualset3
145139	1	409303	5	NULL	NULL	0	NULL	convergence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The convergence of these two trends -- one seeking to distribute responsibility for lifestyle more equitably and the other seeking to distribute responsibility for planning health programs more equitably -- calls for policies , strategies , and interventions that will place similar emphasis on health education and organizational , economic , and environmental supports for health behavior .
	manualset3
145140	2	409303	5	NULL	NULL	0	NULL	two trends	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The convergence of these two trends -- one seeking to distribute responsibility for lifestyle more equitably and the other seeking to distribute responsibility for planning health programs more equitably -- calls for policies , strategies , and interventions that will place similar emphasis on health education and organizational , economic , and environmental supports for health behavior .
	manualset3
145141	3	409303	5	NULL	NULL	0	NULL	one 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The convergence of these two trends -- one seeking to distribute responsibility for lifestyle more equitably and the other seeking to distribute responsibility for planning health programs more equitably -- calls for policies , strategies , and interventions that will place similar emphasis on health education and organizational , economic , and environmental supports for health behavior .
	manualset3
145142	4	409303	5	NULL	NULL	0	NULL	responsibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The convergence of these two trends -- one seeking to distribute responsibility for lifestyle more equitably and the other seeking to distribute responsibility for planning health programs more equitably -- calls for policies , strategies , and interventions that will place similar emphasis on health education and organizational , economic , and environmental supports for health behavior .
	manualset3
145143	5	409303	5	NULL	NULL	0	NULL	lifestyle 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The convergence of these two trends -- one seeking to distribute responsibility for lifestyle more equitably and the other seeking to distribute responsibility for planning health programs more equitably -- calls for policies , strategies , and interventions that will place similar emphasis on health education and organizational , economic , and environmental supports for health behavior .
	manualset3
145144	6	409303	5	NULL	NULL	0	NULL	responsibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The convergence of these two trends -- one seeking to distribute responsibility for lifestyle more equitably and the other seeking to distribute responsibility for planning health programs more equitably -- calls for policies , strategies , and interventions that will place similar emphasis on health education and organizational , economic , and environmental supports for health behavior .
	manualset3
145145	7	409303	5	NULL	NULL	0	NULL	health programs 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The convergence of these two trends -- one seeking to distribute responsibility for lifestyle more equitably and the other seeking to distribute responsibility for planning health programs more equitably -- calls for policies , strategies , and interventions that will place similar emphasis on health education and organizational , economic , and environmental supports for health behavior .
	manualset3
145146	8	409303	5	NULL	NULL	0	NULL	calls 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The convergence of these two trends -- one seeking to distribute responsibility for lifestyle more equitably and the other seeking to distribute responsibility for planning health programs more equitably -- calls for policies , strategies , and interventions that will place similar emphasis on health education and organizational , economic , and environmental supports for health behavior .
	manualset3
145147	9	409303	5	NULL	NULL	0	NULL	policies 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The convergence of these two trends -- one seeking to distribute responsibility for lifestyle more equitably and the other seeking to distribute responsibility for planning health programs more equitably -- calls for policies , strategies , and interventions that will place similar emphasis on health education and organizational , economic , and environmental supports for health behavior .
	manualset3
145148	10	409303	5	NULL	NULL	0	NULL	strategies 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The convergence of these two trends -- one seeking to distribute responsibility for lifestyle more equitably and the other seeking to distribute responsibility for planning health programs more equitably -- calls for policies , strategies , and interventions that will place similar emphasis on health education and organizational , economic , and environmental supports for health behavior .
	manualset3
145149	11	409303	5	NULL	NULL	0	NULL	interventions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The convergence of these two trends -- one seeking to distribute responsibility for lifestyle more equitably and the other seeking to distribute responsibility for planning health programs more equitably -- calls for policies , strategies , and interventions that will place similar emphasis on health education and organizational , economic , and environmental supports for health behavior .
	manualset3
145150	12	409303	5	NULL	NULL	0	NULL	emphasis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The convergence of these two trends -- one seeking to distribute responsibility for lifestyle more equitably and the other seeking to distribute responsibility for planning health programs more equitably -- calls for policies , strategies , and interventions that will place similar emphasis on health education and organizational , economic , and environmental supports for health behavior .
	manualset3
145151	13	409303	5	NULL	NULL	0	NULL	health education	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The convergence of these two trends -- one seeking to distribute responsibility for lifestyle more equitably and the other seeking to distribute responsibility for planning health programs more equitably -- calls for policies , strategies , and interventions that will place similar emphasis on health education and organizational , economic , and environmental supports for health behavior .
	manualset3
145152	14	409303	5	NULL	NULL	0	NULL	organizational supports 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The convergence of these two trends -- one seeking to distribute responsibility for lifestyle more equitably and the other seeking to distribute responsibility for planning health programs more equitably -- calls for policies , strategies , and interventions that will place similar emphasis on health education and organizational , economic , and environmental supports for health behavior .
	manualset3
145153	15	409303	5	NULL	NULL	0	NULL	economic supports 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The convergence of these two trends -- one seeking to distribute responsibility for lifestyle more equitably and the other seeking to distribute responsibility for planning health programs more equitably -- calls for policies , strategies , and interventions that will place similar emphasis on health education and organizational , economic , and environmental supports for health behavior .
	manualset3
145154	16	409303	5	NULL	NULL	0	NULL	environmental supports 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The convergence of these two trends -- one seeking to distribute responsibility for lifestyle more equitably and the other seeking to distribute responsibility for planning health programs more equitably -- calls for policies , strategies , and interventions that will place similar emphasis on health education and organizational , economic , and environmental supports for health behavior .
	manualset3
145155	17	409303	5	NULL	NULL	0	NULL	health behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The convergence of these two trends -- one seeking to distribute responsibility for lifestyle more equitably and the other seeking to distribute responsibility for planning health programs more equitably -- calls for policies , strategies , and interventions that will place similar emphasis on health education and organizational , economic , and environmental supports for health behavior .
	manualset3
145156	1	409304	5	NULL	NULL	0	NULL	conversion rate 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The conversion rate of alpha-TCP and the crystallinity of the formed apatite apparently were not affected by the type of polyester used , but significantly depended on the alpha-TCP content of the composites .
	manualset3
145157	2	409304	5	NULL	NULL	0	NULL	alpha-TCP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The conversion rate of alpha-TCP and the crystallinity of the formed apatite apparently were not affected by the type of polyester used , but significantly depended on the alpha-TCP content of the composites .
	manualset3
145158	3	409304	5	NULL	NULL	0	NULL	crystallinity 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The conversion rate of alpha-TCP and the crystallinity of the formed apatite apparently were not affected by the type of polyester used , but significantly depended on the alpha-TCP content of the composites .
	manualset3
145159	4	409304	5	NULL	NULL	0	NULL	apatite 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The conversion rate of alpha-TCP and the crystallinity of the formed apatite apparently were not affected by the type of polyester used , but significantly depended on the alpha-TCP content of the composites .
	manualset3
145160	5	409304	5	NULL	NULL	0	NULL	type 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The conversion rate of alpha-TCP and the crystallinity of the formed apatite apparently were not affected by the type of polyester used , but significantly depended on the alpha-TCP content of the composites .
	manualset3
145161	6	409304	5	NULL	NULL	0	NULL	polyester 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The conversion rate of alpha-TCP and the crystallinity of the formed apatite apparently were not affected by the type of polyester used , but significantly depended on the alpha-TCP content of the composites .
	manualset3
145162	7	409304	5	NULL	NULL	0	NULL	alpha-TCP content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The conversion rate of alpha-TCP and the crystallinity of the formed apatite apparently were not affected by the type of polyester used , but significantly depended on the alpha-TCP content of the composites .
	manualset3
145163	8	409304	5	NULL	NULL	0	NULL	composites 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The conversion rate of alpha-TCP and the crystallinity of the formed apatite apparently were not affected by the type of polyester used , but significantly depended on the alpha-TCP content of the composites .
	manualset3
145164	1	409305	5	NULL	NULL	0	NULL	coordination structures 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The coordination structures of U ( IV ) , Np ( IV ) , and Th ( IV ) in aqueous solution have been determined by studying the X-ray absorption near edge structure ( XANES ) of the actinide ( An ) L ( 3 ) - edge absorption spectra .
	manualset3
145165	2	409305	5	NULL	NULL	0	NULL	U ( IV )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The coordination structures of U ( IV ) , Np ( IV ) , and Th ( IV ) in aqueous solution have been determined by studying the X-ray absorption near edge structure ( XANES ) of the actinide ( An ) L ( 3 ) - edge absorption spectra .
	manualset3
145166	3	409305	5	NULL	NULL	0	NULL	Np ( IV )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The coordination structures of U ( IV ) , Np ( IV ) , and Th ( IV ) in aqueous solution have been determined by studying the X-ray absorption near edge structure ( XANES ) of the actinide ( An ) L ( 3 ) - edge absorption spectra .
	manualset3
145167	4	409305	5	NULL	NULL	0	NULL	Th ( IV )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The coordination structures of U ( IV ) , Np ( IV ) , and Th ( IV ) in aqueous solution have been determined by studying the X-ray absorption near edge structure ( XANES ) of the actinide ( An ) L ( 3 ) - edge absorption spectra .
	manualset3
145168	5	409305	5	NULL	NULL	0	NULL	aqueous solution 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The coordination structures of U ( IV ) , Np ( IV ) , and Th ( IV ) in aqueous solution have been determined by studying the X-ray absorption near edge structure ( XANES ) of the actinide ( An ) L ( 3 ) - edge absorption spectra .
	manualset3
145169	6	409305	5	NULL	NULL	NULL	NULL	X-ray absorption near edge structure ( XANES )	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The coordination structures of U ( IV ) , Np ( IV ) , and Th ( IV ) in aqueous solution have been determined by studying the X-ray absorption near edge structure ( XANES ) of the actinide ( An ) L ( 3 ) - edge absorption spectra .
	manualset3
145170	7	409305	5	NULL	NULL	0	NULL	actinide ( An ) L ( 3 ) - edge absorption spectra	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The coordination structures of U ( IV ) , Np ( IV ) , and Th ( IV ) in aqueous solution have been determined by studying the X-ray absorption near edge structure ( XANES ) of the actinide ( An ) L ( 3 ) - edge absorption spectra .
	manualset3
145171	1	409306	5	NULL	NULL	0	NULL	copolymer 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The copolymer , which consists of a combination of hydrophobic monomers ( methyl methacrylate ( MMA ) ) and hydrophilic monomers ( vinylpyrolidone ( VP ) ) , have all the required major elements , such as hydrogen , carbon , nitrogen , and oxygen , found in tissues .
	manualset3
145172	2	409306	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The copolymer , which consists of a combination of hydrophobic monomers ( methyl methacrylate ( MMA ) ) and hydrophilic monomers ( vinylpyrolidone ( VP ) ) , have all the required major elements , such as hydrogen , carbon , nitrogen , and oxygen , found in tissues .
	manualset3
145173	3	409306	5	NULL	NULL	0	NULL	hydrophobic monomers ( methyl methacrylate ( MMA ) ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The copolymer , which consists of a combination of hydrophobic monomers ( methyl methacrylate ( MMA ) ) and hydrophilic monomers ( vinylpyrolidone ( VP ) ) , have all the required major elements , such as hydrogen , carbon , nitrogen , and oxygen , found in tissues .
	manualset3
145174	4	409306	5	NULL	NULL	0	NULL	hydrophilic monomers ( vinylpyrolidone ( VP ) ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The copolymer , which consists of a combination of hydrophobic monomers ( methyl methacrylate ( MMA ) ) and hydrophilic monomers ( vinylpyrolidone ( VP ) ) , have all the required major elements , such as hydrogen , carbon , nitrogen , and oxygen , found in tissues .
	manualset3
145175	5	409306	5	NULL	NULL	0	NULL	elements 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The copolymer , which consists of a combination of hydrophobic monomers ( methyl methacrylate ( MMA ) ) and hydrophilic monomers ( vinylpyrolidone ( VP ) ) , have all the required major elements , such as hydrogen , carbon , nitrogen , and oxygen , found in tissues .
	manualset3
145176	6	409306	5	NULL	NULL	0	NULL	hydrogen 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The copolymer , which consists of a combination of hydrophobic monomers ( methyl methacrylate ( MMA ) ) and hydrophilic monomers ( vinylpyrolidone ( VP ) ) , have all the required major elements , such as hydrogen , carbon , nitrogen , and oxygen , found in tissues .
	manualset3
145177	7	409306	5	NULL	NULL	0	NULL	carbon 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The copolymer , which consists of a combination of hydrophobic monomers ( methyl methacrylate ( MMA ) ) and hydrophilic monomers ( vinylpyrolidone ( VP ) ) , have all the required major elements , such as hydrogen , carbon , nitrogen , and oxygen , found in tissues .
	manualset3
145178	8	409306	5	NULL	NULL	0	NULL	nitrogen 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The copolymer , which consists of a combination of hydrophobic monomers ( methyl methacrylate ( MMA ) ) and hydrophilic monomers ( vinylpyrolidone ( VP ) ) , have all the required major elements , such as hydrogen , carbon , nitrogen , and oxygen , found in tissues .
	manualset3
145179	9	409306	5	NULL	NULL	0	NULL	oxygen 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The copolymer , which consists of a combination of hydrophobic monomers ( methyl methacrylate ( MMA ) ) and hydrophilic monomers ( vinylpyrolidone ( VP ) ) , have all the required major elements , such as hydrogen , carbon , nitrogen , and oxygen , found in tissues .
	manualset3
145180	10	409306	5	NULL	NULL	0	NULL	tissues 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The copolymer , which consists of a combination of hydrophobic monomers ( methyl methacrylate ( MMA ) ) and hydrophilic monomers ( vinylpyrolidone ( VP ) ) , have all the required major elements , such as hydrogen , carbon , nitrogen , and oxygen , found in tissues .
	manualset3
145181	1	409307	5	NULL	NULL	0	NULL	core clostripain protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The core clostripain protein fused to the PGA signal peptide was also prepared .
	manualset3
145182	2	409307	5	NULL	NULL	0	NULL	PGA signal peptide 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The core clostripain protein fused to the PGA signal peptide was also prepared .
	manualset3
145183	1	409308	5	NULL	NULL	0	NULL	significant right ear advantage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant right ear advantage was not obtained in the divided attention condition due to a ceiling effect .
	manualset3
145184	2	409308	5	NULL	NULL	0	NULL	divided attention condition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant right ear advantage was not obtained in the divided attention condition due to a ceiling effect .
	manualset3
145185	3	409308	5	NULL	NULL	0	NULL	ceiling effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A significant right ear advantage was not obtained in the divided attention condition due to a ceiling effect .
	manualset3
145186	1	409309	5	NULL	NULL	0	NULL	corneal epithelium	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The corneal epithelium healed , conjunctival-scleral necrosis resolved completely and the visual acuity improved to 6/36 in the right eye after 3 months of immunosuppressive therapy .
	manualset3
145187	2	409309	5	NULL	NULL	0	NULL	conjunctival-scleral necrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The corneal epithelium healed , conjunctival-scleral necrosis resolved completely and the visual acuity improved to 6/36 in the right eye after 3 months of immunosuppressive therapy .
	manualset3
145188	3	409309	5	NULL	NULL	0	NULL	visual acuity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The corneal epithelium healed , conjunctival-scleral necrosis resolved completely and the visual acuity improved to 6/36 in the right eye after 3 months of immunosuppressive therapy .
	manualset3
145190	4	409309	5	NULL	NULL	0	NULL	6/36 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The corneal epithelium healed , conjunctival-scleral necrosis resolved completely and the visual acuity improved to 6/36 in the right eye after 3 months of immunosuppressive therapy .
	manualset3
145191	5	409309	5	NULL	NULL	0	NULL	right eye 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The corneal epithelium healed , conjunctival-scleral necrosis resolved completely and the visual acuity improved to 6/36 in the right eye after 3 months of immunosuppressive therapy .
	manualset3
145192	6	409309	5	NULL	NULL	0	NULL	3 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The corneal epithelium healed , conjunctival-scleral necrosis resolved completely and the visual acuity improved to 6/36 in the right eye after 3 months of immunosuppressive therapy .
	manualset3
145193	7	409309	5	NULL	NULL	0	NULL	immunosuppressive therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The corneal epithelium healed , conjunctival-scleral necrosis resolved completely and the visual acuity improved to 6/36 in the right eye after 3 months of immunosuppressive therapy .
	manualset3
145194	1	409310	5	NULL	NULL	0	NULL	correct clinical assessment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The correct clinical assessment and treatment of such cases require the attention of a team comprising a neurosurgeon , ophthalmologist , otolaryngologist , and plastic surgeon .
	manualset3
145195	2	409310	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The correct clinical assessment and treatment of such cases require the attention of a team comprising a neurosurgeon , ophthalmologist , otolaryngologist , and plastic surgeon .
	manualset3
145196	3	409310	5	NULL	NULL	0	NULL	cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The correct clinical assessment and treatment of such cases require the attention of a team comprising a neurosurgeon , ophthalmologist , otolaryngologist , and plastic surgeon .
	manualset3
145197	4	409310	5	NULL	NULL	0	NULL	attention 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The correct clinical assessment and treatment of such cases require the attention of a team comprising a neurosurgeon , ophthalmologist , otolaryngologist , and plastic surgeon .
	manualset3
145198	5	409310	5	NULL	NULL	0	NULL	team 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The correct clinical assessment and treatment of such cases require the attention of a team comprising a neurosurgeon , ophthalmologist , otolaryngologist , and plastic surgeon .
	manualset3
145199	6	409310	5	NULL	NULL	0	NULL	neurosurgeon 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The correct clinical assessment and treatment of such cases require the attention of a team comprising a neurosurgeon , ophthalmologist , otolaryngologist , and plastic surgeon .
	manualset3
145200	7	409310	5	NULL	NULL	0	NULL	ophthalmologist 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The correct clinical assessment and treatment of such cases require the attention of a team comprising a neurosurgeon , ophthalmologist , otolaryngologist , and plastic surgeon .
	manualset3
145201	8	409310	5	NULL	NULL	0	NULL	otolaryngologist 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The correct clinical assessment and treatment of such cases require the attention of a team comprising a neurosurgeon , ophthalmologist , otolaryngologist , and plastic surgeon .
	manualset3
145202	9	409310	5	NULL	NULL	0	NULL	plastic surgeon	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The correct clinical assessment and treatment of such cases require the attention of a team comprising a neurosurgeon , ophthalmologist , otolaryngologist , and plastic surgeon .
	manualset3
145203	1	409311	5	NULL	NULL	NULL	NULL	recognition 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The correct recognition of spondyloarthritides is essential in order to identify common therapeutic strategies , especially in the era of new biological therapies such as infliximab .
	manualset3
145204	2	409311	5	NULL	NULL	0	NULL	spondyloarthritides 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The correct recognition of spondyloarthritides is essential in order to identify common therapeutic strategies , especially in the era of new biological therapies such as infliximab .
	manualset3
145205	3	409311	5	NULL	NULL	0	NULL	common therapeutic strategies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The correct recognition of spondyloarthritides is essential in order to identify common therapeutic strategies , especially in the era of new biological therapies such as infliximab .
	manualset3
145206	4	409311	5	NULL	NULL	0	NULL	era 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The correct recognition of spondyloarthritides is essential in order to identify common therapeutic strategies , especially in the era of new biological therapies such as infliximab .
	manualset3
145207	5	409311	5	NULL	NULL	0	NULL	new biological therapies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The correct recognition of spondyloarthritides is essential in order to identify common therapeutic strategies , especially in the era of new biological therapies such as infliximab .
	manualset3
145208	6	409311	5	NULL	NULL	0	NULL	infliximab 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The correct recognition of spondyloarthritides is essential in order to identify common therapeutic strategies , especially in the era of new biological therapies such as infliximab .
	manualset3
145209	1	409312	5	NULL	NULL	0	NULL	correlation coefficients 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation coefficients between DRSC and the total polyphenol or total catechin content of the tea infusions were 1.0 and 0.99 .
	manualset3
145210	2	409312	5	NULL	NULL	0	NULL	DRSC 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation coefficients between DRSC and the total polyphenol or total catechin content of the tea infusions were 1.0 and 0.99 .
	manualset3
145211	3	409312	5	NULL	NULL	0	NULL	total polyphenol 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation coefficients between DRSC and the total polyphenol or total catechin content of the tea infusions were 1.0 and 0.99 .
	manualset3
145212	4	409312	5	NULL	NULL	0	NULL	total catechin content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation coefficients between DRSC and the total polyphenol or total catechin content of the tea infusions were 1.0 and 0.99 .
	manualset3
145213	5	409312	5	NULL	NULL	0	NULL	tea infusions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation coefficients between DRSC and the total polyphenol or total catechin content of the tea infusions were 1.0 and 0.99 .
	manualset3
145214	6	409312	5	NULL	NULL	0	NULL	1.0 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation coefficients between DRSC and the total polyphenol or total catechin content of the tea infusions were 1.0 and 0.99 .
	manualset3
145215	7	409312	5	NULL	NULL	0	NULL	0.99 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation coefficients between DRSC and the total polyphenol or total catechin content of the tea infusions were 1.0 and 0.99 .
	manualset3
145216	1	409313	5	NULL	NULL	0	NULL	correlation coefficients 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation coefficients were generally higher for zone `` Beta , '' characterized by complete chorioretinal atrophy with visible large choroidal vessels and sclera , than for zone `` Alpha , '' which showed irregular hypo - and hyperpigmentation .
	manualset3
145217	2	409313	5	NULL	NULL	NULL	NULL	zone `` Beta , ''	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The correlation coefficients were generally higher for zone `` Beta , '' characterized by complete chorioretinal atrophy with visible large choroidal vessels and sclera , than for zone `` Alpha , '' which showed irregular hypo - and hyperpigmentation .
	manualset3
145218	3	409313	5	NULL	NULL	0	NULL	complete chorioretinal atrophy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation coefficients were generally higher for zone `` Beta , '' characterized by complete chorioretinal atrophy with visible large choroidal vessels and sclera , than for zone `` Alpha , '' which showed irregular hypo - and hyperpigmentation .
	manualset3
145219	4	409313	5	NULL	NULL	0	NULL	visible large choroidal vessels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation coefficients were generally higher for zone `` Beta , '' characterized by complete chorioretinal atrophy with visible large choroidal vessels and sclera , than for zone `` Alpha , '' which showed irregular hypo - and hyperpigmentation .
	manualset3
145220	5	409313	5	NULL	NULL	0	NULL	sclera 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation coefficients were generally higher for zone `` Beta , '' characterized by complete chorioretinal atrophy with visible large choroidal vessels and sclera , than for zone `` Alpha , '' which showed irregular hypo - and hyperpigmentation .
	manualset3
145221	6	409313	5	NULL	NULL	0	NULL	zone `` Alpha , ''	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation coefficients were generally higher for zone `` Beta , '' characterized by complete chorioretinal atrophy with visible large choroidal vessels and sclera , than for zone `` Alpha , '' which showed irregular hypo - and hyperpigmentation .
	manualset3
145222	7	409313	5	NULL	NULL	0	NULL	hypopigmentation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation coefficients were generally higher for zone `` Beta , '' characterized by complete chorioretinal atrophy with visible large choroidal vessels and sclera , than for zone `` Alpha , '' which showed irregular hypo - and hyperpigmentation .
	manualset3
145223	8	409313	5	NULL	NULL	0	NULL	hyperpigmentation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation coefficients were generally higher for zone `` Beta , '' characterized by complete chorioretinal atrophy with visible large choroidal vessels and sclera , than for zone `` Alpha , '' which showed irregular hypo - and hyperpigmentation .
	manualset3
145224	1	409314	5	NULL	NULL	0	NULL	correlation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation of genetic and biochemical complementation argues that Sir2p trimerization is physiologically relevant for rDNA silencing .
	manualset3
145225	2	409314	5	NULL	NULL	0	NULL	genetic complementation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation of genetic and biochemical complementation argues that Sir2p trimerization is physiologically relevant for rDNA silencing .
	manualset3
145226	3	409314	5	NULL	NULL	0	NULL	biochemical complementation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation of genetic and biochemical complementation argues that Sir2p trimerization is physiologically relevant for rDNA silencing .
	manualset3
145227	4	409314	5	NULL	NULL	0	NULL	Sir2p trimerization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation of genetic and biochemical complementation argues that Sir2p trimerization is physiologically relevant for rDNA silencing .
	manualset3
145228	5	409314	5	NULL	NULL	0	NULL	rDNA silencing	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation of genetic and biochemical complementation argues that Sir2p trimerization is physiologically relevant for rDNA silencing .
	manualset3
145229	1	409315	5	NULL	NULL	0	NULL	correlation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation was found between the level of AAB to NGF and the degree of disease progression .
	manualset3
145230	2	409315	5	NULL	NULL	0	NULL	level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation was found between the level of AAB to NGF and the degree of disease progression .
	manualset3
145231	3	409315	5	NULL	NULL	0	NULL	AAB 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation was found between the level of AAB to NGF and the degree of disease progression .
	manualset3
145232	4	409315	5	NULL	NULL	0	NULL	NGF 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation was found between the level of AAB to NGF and the degree of disease progression .
	manualset3
145233	5	409315	5	NULL	NULL	0	NULL	degree 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation was found between the level of AAB to NGF and the degree of disease progression .
	manualset3
145234	6	409315	5	NULL	NULL	0	NULL	disease progression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation was found between the level of AAB to NGF and the degree of disease progression .
	manualset3
145235	1	409316	5	NULL	NULL	0	NULL	correlation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation was not improved by expressing DPA in different dimensions , but was improved by including normal women .
	manualset3
145236	2	409316	5	NULL	NULL	0	NULL	DPA 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation was not improved by expressing DPA in different dimensions , but was improved by including normal women .
	manualset3
145237	3	409316	5	NULL	NULL	0	NULL	dimensions 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation was not improved by expressing DPA in different dimensions , but was improved by including normal women .
	manualset3
145238	4	409316	5	NULL	NULL	0	NULL	normal women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation was not improved by expressing DPA in different dimensions , but was improved by including normal women .
	manualset3
145239	1	409317	5	NULL	NULL	0	NULL	correlations 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlations between surface phenotype , rearrangement of TRG gamma , TCR beta , and Ig H chain genes were analyzed .
	manualset3
145240	2	409317	5	NULL	NULL	0	NULL	surface phenotype	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlations between surface phenotype , rearrangement of TRG gamma , TCR beta , and Ig H chain genes were analyzed .
	manualset3
145241	3	409317	5	NULL	NULL	0	NULL	rearrangement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlations between surface phenotype , rearrangement of TRG gamma , TCR beta , and Ig H chain genes were analyzed .
	manualset3
145242	4	409317	5	NULL	NULL	NULL	NULL	TRG gamma	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The correlations between surface phenotype , rearrangement of TRG gamma , TCR beta , and Ig H chain genes were analyzed .
	manualset3
145243	5	409317	5	NULL	NULL	0	NULL	TCR beta	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlations between surface phenotype , rearrangement of TRG gamma , TCR beta , and Ig H chain genes were analyzed .
	manualset3
145244	6	409317	5	NULL	NULL	0	NULL	Ig H chain gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlations between surface phenotype , rearrangement of TRG gamma , TCR beta , and Ig H chain genes were analyzed .
	manualset3
145245	1	409318	5	NULL	NULL	0	NULL	silent revolution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A silent revolution -- changes in maternity ward routines with regard to infant feeding in Norway 1973-1982 .
	manualset3
145246	2	409318	5	NULL	NULL	0	NULL	maternity ward routines	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A silent revolution -- changes in maternity ward routines with regard to infant feeding in Norway 1973-1982 .
	manualset3
145247	3	409318	5	NULL	NULL	0	NULL	infant feeding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A silent revolution -- changes in maternity ward routines with regard to infant feeding in Norway 1973-1982 .
	manualset3
145248	4	409318	5	NULL	NULL	0	NULL	Norway 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A silent revolution -- changes in maternity ward routines with regard to infant feeding in Norway 1973-1982 .
	manualset3
145249	5	409318	5	NULL	NULL	0	NULL	1973-1982	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A silent revolution -- changes in maternity ward routines with regard to infant feeding in Norway 1973-1982 .
	manualset3
145250	1	409319	5	NULL	NULL	0	NULL	average pH values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The corresponding average pH values were 5.86 for A549 , 6.00 for H1299 , 6.20 for CH27 , 6.90 for BEAS-2B , 6.96 for MRC5 , and 7.02 for WI38 , respectively , after the cells were completely adhered to the PSW surface .
	manualset3
145251	2	409319	5	NULL	NULL	0	NULL	5.86	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The corresponding average pH values were 5.86 for A549 , 6.00 for H1299 , 6.20 for CH27 , 6.90 for BEAS-2B , 6.96 for MRC5 , and 7.02 for WI38 , respectively , after the cells were completely adhered to the PSW surface .
	manualset3
145252	3	409319	5	NULL	NULL	0	NULL	A549 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The corresponding average pH values were 5.86 for A549 , 6.00 for H1299 , 6.20 for CH27 , 6.90 for BEAS-2B , 6.96 for MRC5 , and 7.02 for WI38 , respectively , after the cells were completely adhered to the PSW surface .
	manualset3
145253	4	409319	5	NULL	NULL	0	NULL	6.00 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The corresponding average pH values were 5.86 for A549 , 6.00 for H1299 , 6.20 for CH27 , 6.90 for BEAS-2B , 6.96 for MRC5 , and 7.02 for WI38 , respectively , after the cells were completely adhered to the PSW surface .
	manualset3
145254	5	409319	5	NULL	NULL	0	NULL	H1299 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The corresponding average pH values were 5.86 for A549 , 6.00 for H1299 , 6.20 for CH27 , 6.90 for BEAS-2B , 6.96 for MRC5 , and 7.02 for WI38 , respectively , after the cells were completely adhered to the PSW surface .
	manualset3
145255	6	409319	5	NULL	NULL	0	NULL	6.20 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The corresponding average pH values were 5.86 for A549 , 6.00 for H1299 , 6.20 for CH27 , 6.90 for BEAS-2B , 6.96 for MRC5 , and 7.02 for WI38 , respectively , after the cells were completely adhered to the PSW surface .
	manualset3
145256	7	409319	5	NULL	NULL	0	NULL	CH27 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The corresponding average pH values were 5.86 for A549 , 6.00 for H1299 , 6.20 for CH27 , 6.90 for BEAS-2B , 6.96 for MRC5 , and 7.02 for WI38 , respectively , after the cells were completely adhered to the PSW surface .
	manualset3
145257	8	409319	5	NULL	NULL	0	NULL	6.90 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The corresponding average pH values were 5.86 for A549 , 6.00 for H1299 , 6.20 for CH27 , 6.90 for BEAS-2B , 6.96 for MRC5 , and 7.02 for WI38 , respectively , after the cells were completely adhered to the PSW surface .
	manualset3
145258	9	409319	5	NULL	NULL	0	NULL	BEAS-2B	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The corresponding average pH values were 5.86 for A549 , 6.00 for H1299 , 6.20 for CH27 , 6.90 for BEAS-2B , 6.96 for MRC5 , and 7.02 for WI38 , respectively , after the cells were completely adhered to the PSW surface .
	manualset3
145259	10	409319	5	NULL	NULL	0	NULL	6.96 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The corresponding average pH values were 5.86 for A549 , 6.00 for H1299 , 6.20 for CH27 , 6.90 for BEAS-2B , 6.96 for MRC5 , and 7.02 for WI38 , respectively , after the cells were completely adhered to the PSW surface .
	manualset3
145260	11	409319	5	NULL	NULL	0	NULL	MRC5 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The corresponding average pH values were 5.86 for A549 , 6.00 for H1299 , 6.20 for CH27 , 6.90 for BEAS-2B , 6.96 for MRC5 , and 7.02 for WI38 , respectively , after the cells were completely adhered to the PSW surface .
	manualset3
145261	12	409319	5	NULL	NULL	0	NULL	 7.02	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The corresponding average pH values were 5.86 for A549 , 6.00 for H1299 , 6.20 for CH27 , 6.90 for BEAS-2B , 6.96 for MRC5 , and 7.02 for WI38 , respectively , after the cells were completely adhered to the PSW surface .
	manualset3
145262	13	409319	5	NULL	NULL	0	NULL	WI38 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The corresponding average pH values were 5.86 for A549 , 6.00 for H1299 , 6.20 for CH27 , 6.90 for BEAS-2B , 6.96 for MRC5 , and 7.02 for WI38 , respectively , after the cells were completely adhered to the PSW surface .
	manualset3
145263	14	409319	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The corresponding average pH values were 5.86 for A549 , 6.00 for H1299 , 6.20 for CH27 , 6.90 for BEAS-2B , 6.96 for MRC5 , and 7.02 for WI38 , respectively , after the cells were completely adhered to the PSW surface .
	manualset3
145264	15	409319	5	NULL	NULL	0	NULL	PSW surface	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The corresponding average pH values were 5.86 for A549 , 6.00 for H1299 , 6.20 for CH27 , 6.90 for BEAS-2B , 6.96 for MRC5 , and 7.02 for WI38 , respectively , after the cells were completely adhered to the PSW surface .
	manualset3
145265	1	409320	5	NULL	NULL	0	NULL	enzyme concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The corresponding enzyme concentration in the crude homogenates was calculated and corresponded well with the number of ( 3H ) ouabain binding sites measured in intact muscles or biopsies hereof .
	manualset3
145266	2	409320	5	NULL	NULL	0	NULL	crude homogenates	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The corresponding enzyme concentration in the crude homogenates was calculated and corresponded well with the number of ( 3H ) ouabain binding sites measured in intact muscles or biopsies hereof .
	manualset3
145267	3	409320	5	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The corresponding enzyme concentration in the crude homogenates was calculated and corresponded well with the number of ( 3H ) ouabain binding sites measured in intact muscles or biopsies hereof .
	manualset3
145268	4	409320	5	NULL	NULL	0	NULL	( 3H ) ouabain binding sites	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The corresponding enzyme concentration in the crude homogenates was calculated and corresponded well with the number of ( 3H ) ouabain binding sites measured in intact muscles or biopsies hereof .
	manualset3
145269	5	409320	5	NULL	NULL	0	NULL	intact muscles	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The corresponding enzyme concentration in the crude homogenates was calculated and corresponded well with the number of ( 3H ) ouabain binding sites measured in intact muscles or biopsies hereof .
	manualset3
145270	6	409320	5	NULL	NULL	0	NULL	biopsies 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The corresponding enzyme concentration in the crude homogenates was calculated and corresponded well with the number of ( 3H ) ouabain binding sites measured in intact muscles or biopsies hereof .
	manualset3
148668	7	409320	5	NULL	NULL	0	NULL	well	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The corresponding enzyme concentration in the crude homogenates was calculated and corresponded well with the number of ( 3H ) ouabain binding sites measured in intact muscles or biopsies hereof .
	manualset3
145271	1	409321	5	NULL	NULL	0	NULL	numbers 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The corresponding numbers for exposure to quartz were halved and lost their statistical significance when the misclassification was allowed for .
	manualset3
145272	2	409321	5	NULL	NULL	0	NULL	exposure 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The corresponding numbers for exposure to quartz were halved and lost their statistical significance when the misclassification was allowed for .
	manualset3
145273	3	409321	5	NULL	NULL	0	NULL	quartz 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The corresponding numbers for exposure to quartz were halved and lost their statistical significance when the misclassification was allowed for .
	manualset3
145274	4	409321	5	NULL	NULL	0	NULL	statistical significance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The corresponding numbers for exposure to quartz were halved and lost their statistical significance when the misclassification was allowed for .
	manualset3
145275	5	409321	5	NULL	NULL	0	NULL	misclassification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The corresponding numbers for exposure to quartz were halved and lost their statistical significance when the misclassification was allowed for .
	manualset3
145276	1	409322	5	NULL	NULL	0	NULL	cortical malformation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cortical malformation is interpreted with regard to developmental mechanisms , and observations from a mouse model of TD .
	manualset3
145277	2	409322	5	NULL	NULL	0	NULL	developmental mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cortical malformation is interpreted with regard to developmental mechanisms , and observations from a mouse model of TD .
	manualset3
145278	3	409322	5	NULL	NULL	0	NULL	observations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cortical malformation is interpreted with regard to developmental mechanisms , and observations from a mouse model of TD .
	manualset3
145279	4	409322	5	NULL	NULL	0	NULL	mouse model	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The cortical malformation is interpreted with regard to developmental mechanisms , and observations from a mouse model of TD .
	manualset3
145280	5	409322	5	NULL	NULL	0	NULL	TD 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The cortical malformation is interpreted with regard to developmental mechanisms , and observations from a mouse model of TD .
	manualset3
145281	1	409323	5	NULL	NULL	0	NULL	cortical rhythmic changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cortical rhythmic changes were distinct in the singing condition compared with the other vocalizing conditions ( speaking and humming ) and thus we considered that more concentrated control of the vocal tract , diaphragm and abdominal muscles is responsible .
	manualset3
145282	2	409323	5	NULL	NULL	0	NULL	singing condition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cortical rhythmic changes were distinct in the singing condition compared with the other vocalizing conditions ( speaking and humming ) and thus we considered that more concentrated control of the vocal tract , diaphragm and abdominal muscles is responsible .
	manualset3
145283	3	409323	5	NULL	NULL	0	NULL	vocalizing conditions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cortical rhythmic changes were distinct in the singing condition compared with the other vocalizing conditions ( speaking and humming ) and thus we considered that more concentrated control of the vocal tract , diaphragm and abdominal muscles is responsible .
	manualset3
145284	4	409323	5	NULL	NULL	0	NULL	speaking 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cortical rhythmic changes were distinct in the singing condition compared with the other vocalizing conditions ( speaking and humming ) and thus we considered that more concentrated control of the vocal tract , diaphragm and abdominal muscles is responsible .
	manualset3
145285	5	409323	5	NULL	NULL	0	NULL	humming 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cortical rhythmic changes were distinct in the singing condition compared with the other vocalizing conditions ( speaking and humming ) and thus we considered that more concentrated control of the vocal tract , diaphragm and abdominal muscles is responsible .
	manualset3
145286	6	409323	5	NULL	NULL	0	NULL	concentrated control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cortical rhythmic changes were distinct in the singing condition compared with the other vocalizing conditions ( speaking and humming ) and thus we considered that more concentrated control of the vocal tract , diaphragm and abdominal muscles is responsible .
	manualset3
145287	7	409323	5	NULL	NULL	0	NULL	vocal tract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The cortical rhythmic changes were distinct in the singing condition compared with the other vocalizing conditions ( speaking and humming ) and thus we considered that more concentrated control of the vocal tract , diaphragm and abdominal muscles is responsible .
	manualset3
145288	8	409323	5	NULL	NULL	0	NULL	diaphragm 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The cortical rhythmic changes were distinct in the singing condition compared with the other vocalizing conditions ( speaking and humming ) and thus we considered that more concentrated control of the vocal tract , diaphragm and abdominal muscles is responsible .
	manualset3
145289	9	409323	5	NULL	NULL	0	NULL	abdominal muscles 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The cortical rhythmic changes were distinct in the singing condition compared with the other vocalizing conditions ( speaking and humming ) and thus we considered that more concentrated control of the vocal tract , diaphragm and abdominal muscles is responsible .
	manualset3
145290	1	409324	5	NULL	NULL	0	NULL	corticotectal projection 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The corticotectal projection of the rat in vitro : development , anatomy and physiological characteristics .
	manualset3
145291	2	409324	5	NULL	NULL	0	NULL	rat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The corticotectal projection of the rat in vitro : development , anatomy and physiological characteristics .
	manualset3
145292	3	409324	5	NULL	NULL	0	NULL	development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The corticotectal projection of the rat in vitro : development , anatomy and physiological characteristics .
	manualset3
145293	4	409324	5	NULL	NULL	0	NULL	anatomy 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The corticotectal projection of the rat in vitro : development , anatomy and physiological characteristics .
	manualset3
145294	5	409324	5	NULL	NULL	0	NULL	physiological characteristics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The corticotectal projection of the rat in vitro : development , anatomy and physiological characteristics .
	manualset3
145295	1	409325	5	NULL	NULL	0	NULL	pattern 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar , but less pronounced , pattern of changes in IGFBP-3 mRNA was seen , whereas levels of IGFBP-6 mRNA were unchanged throughout .
	manualset3
145296	2	409325	5	NULL	NULL	0	NULL	changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar , but less pronounced , pattern of changes in IGFBP-3 mRNA was seen , whereas levels of IGFBP-6 mRNA were unchanged throughout .
	manualset3
145297	3	409325	5	NULL	NULL	0	NULL	IGFBP-3 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar , but less pronounced , pattern of changes in IGFBP-3 mRNA was seen , whereas levels of IGFBP-6 mRNA were unchanged throughout .
	manualset3
145298	4	409325	5	NULL	NULL	0	NULL	levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar , but less pronounced , pattern of changes in IGFBP-3 mRNA was seen , whereas levels of IGFBP-6 mRNA were unchanged throughout .
	manualset3
145299	5	409325	5	NULL	NULL	0	NULL	IGFBP-6 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar , but less pronounced , pattern of changes in IGFBP-3 mRNA was seen , whereas levels of IGFBP-6 mRNA were unchanged throughout .
	manualset3
145300	1	409326	5	NULL	NULL	0	NULL	cosN sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The cosN sequence is bisected by an axis of hyphenated twofold rotational symmetry .
	manualset3
145301	2	409326	5	NULL	NULL	0	NULL	axis of hyphenated twofold rotational symmetry	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cosN sequence is bisected by an axis of hyphenated twofold rotational symmetry .
	manualset3
145302	1	409327	5	NULL	NULL	0	NULL	cosmid clone E. coli K-12 ( pANN801 )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The cosmid clone E. coli K-12 ( pANN801 ) and another nine independently isolated Mrh + cosmid clones derived from a cosmid gene bank of strain 536 express the 16.5-kilodalton protein band , but not the 22-kilodalton protein , indicating an association of the Mrh + property with the `` 16.5-kilodalton fimbriae . ''
	manualset3
145303	2	409327	5	NULL	NULL	0	NULL	nine 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The cosmid clone E. coli K-12 ( pANN801 ) and another nine independently isolated Mrh + cosmid clones derived from a cosmid gene bank of strain 536 express the 16.5-kilodalton protein band , but not the 22-kilodalton protein , indicating an association of the Mrh + property with the `` 16.5-kilodalton fimbriae . ''
	manualset3
145304	3	409327	5	NULL	NULL	NULL	NULL	Mrh + cosmid clones 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The cosmid clone E. coli K-12 ( pANN801 ) and another nine independently isolated Mrh + cosmid clones derived from a cosmid gene bank of strain 536 express the 16.5-kilodalton protein band , but not the 22-kilodalton protein , indicating an association of the Mrh + property with the `` 16.5-kilodalton fimbriae . ''
	manualset3
145305	4	409327	5	NULL	NULL	0	NULL	cosmid gene bank	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The cosmid clone E. coli K-12 ( pANN801 ) and another nine independently isolated Mrh + cosmid clones derived from a cosmid gene bank of strain 536 express the 16.5-kilodalton protein band , but not the 22-kilodalton protein , indicating an association of the Mrh + property with the `` 16.5-kilodalton fimbriae . ''
	manualset3
145306	5	409327	5	NULL	NULL	0	NULL	strain 536	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The cosmid clone E. coli K-12 ( pANN801 ) and another nine independently isolated Mrh + cosmid clones derived from a cosmid gene bank of strain 536 express the 16.5-kilodalton protein band , but not the 22-kilodalton protein , indicating an association of the Mrh + property with the `` 16.5-kilodalton fimbriae . ''
	manualset3
145307	6	409327	5	NULL	NULL	0	NULL	16.5-kilodalton protein band	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The cosmid clone E. coli K-12 ( pANN801 ) and another nine independently isolated Mrh + cosmid clones derived from a cosmid gene bank of strain 536 express the 16.5-kilodalton protein band , but not the 22-kilodalton protein , indicating an association of the Mrh + property with the `` 16.5-kilodalton fimbriae . ''
	manualset3
145308	7	409327	5	NULL	NULL	0	NULL	22-kilodalton protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The cosmid clone E. coli K-12 ( pANN801 ) and another nine independently isolated Mrh + cosmid clones derived from a cosmid gene bank of strain 536 express the 16.5-kilodalton protein band , but not the 22-kilodalton protein , indicating an association of the Mrh + property with the `` 16.5-kilodalton fimbriae . ''
	manualset3
145309	8	409327	5	NULL	NULL	0	NULL	association 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cosmid clone E. coli K-12 ( pANN801 ) and another nine independently isolated Mrh + cosmid clones derived from a cosmid gene bank of strain 536 express the 16.5-kilodalton protein band , but not the 22-kilodalton protein , indicating an association of the Mrh + property with the `` 16.5-kilodalton fimbriae . ''
	manualset3
145310	9	409327	5	NULL	NULL	0	NULL	Mrh + property	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cosmid clone E. coli K-12 ( pANN801 ) and another nine independently isolated Mrh + cosmid clones derived from a cosmid gene bank of strain 536 express the 16.5-kilodalton protein band , but not the 22-kilodalton protein , indicating an association of the Mrh + property with the `` 16.5-kilodalton fimbriae . ''
	manualset3
145311	10	409327	5	NULL	NULL	0	NULL	16.5-kilodalton fimbriae	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The cosmid clone E. coli K-12 ( pANN801 ) and another nine independently isolated Mrh + cosmid clones derived from a cosmid gene bank of strain 536 express the 16.5-kilodalton protein band , but not the 22-kilodalton protein , indicating an association of the Mrh + property with the `` 16.5-kilodalton fimbriae . ''
	manualset3
145312	1	409328	5	NULL	NULL	0	NULL	costs 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The costs and outcomes of treating a deep pressure ulcer in a patient with quadriplegia .
	manualset3
145313	2	409328	5	NULL	NULL	0	NULL	outcomes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The costs and outcomes of treating a deep pressure ulcer in a patient with quadriplegia .
	manualset3
145314	3	409328	5	NULL	NULL	NULL	NULL	deep pressure ulcer	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The costs and outcomes of treating a deep pressure ulcer in a patient with quadriplegia .
	manualset3
145315	4	409328	5	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The costs and outcomes of treating a deep pressure ulcer in a patient with quadriplegia .
	manualset3
145316	5	409328	5	NULL	NULL	0	NULL	quadriplegia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The costs and outcomes of treating a deep pressure ulcer in a patient with quadriplegia .
	manualset3
145317	1	409329	5	NULL	NULL	0	NULL	costs 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The costs of heliotherapy exceeded manyfold the mean monthly cost of conventional psoriasis therapy .
	manualset3
145318	2	409329	5	NULL	NULL	0	NULL	heliotherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The costs of heliotherapy exceeded manyfold the mean monthly cost of conventional psoriasis therapy .
	manualset3
145319	3	409329	5	NULL	NULL	0	NULL	mean monthly cost	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The costs of heliotherapy exceeded manyfold the mean monthly cost of conventional psoriasis therapy .
	manualset3
145320	4	409329	5	NULL	NULL	0	NULL	conventional psoriasis therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The costs of heliotherapy exceeded manyfold the mean monthly cost of conventional psoriasis therapy .
	manualset3
145321	1	409330	5	NULL	NULL	0	NULL	coupling mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The coupling mechanism of sarcoplasmic reticulum ATPase is based on the reciprocal influence of calcium binding and phosphorylation domains .
	manualset3
145322	2	409330	5	NULL	NULL	0	NULL	sarcoplasmic reticulum ATPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The coupling mechanism of sarcoplasmic reticulum ATPase is based on the reciprocal influence of calcium binding and phosphorylation domains .
	manualset3
145323	3	409330	5	NULL	NULL	0	NULL	reciprocal influence	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The coupling mechanism of sarcoplasmic reticulum ATPase is based on the reciprocal influence of calcium binding and phosphorylation domains .
	manualset3
145324	4	409330	5	NULL	NULL	0	NULL	calcium binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The coupling mechanism of sarcoplasmic reticulum ATPase is based on the reciprocal influence of calcium binding and phosphorylation domains .
	manualset3
145325	5	409330	5	NULL	NULL	0	NULL	phosphorylation domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The coupling mechanism of sarcoplasmic reticulum ATPase is based on the reciprocal influence of calcium binding and phosphorylation domains .
	manualset3
145326	1	409331	5	NULL	NULL	0	NULL	course 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The course was web-based and included synchronous and asynchronous communication , on-line libraries and multimedia material .
	manualset3
145327	2	409331	5	NULL	NULL	0	NULL	synchronous communication 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The course was web-based and included synchronous and asynchronous communication , on-line libraries and multimedia material .
	manualset3
145328	3	409331	5	NULL	NULL	0	NULL	asynchronous communication 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The course was web-based and included synchronous and asynchronous communication , on-line libraries and multimedia material .
	manualset3
145329	4	409331	5	NULL	NULL	0	NULL	on-line libraries	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The course was web-based and included synchronous and asynchronous communication , on-line libraries and multimedia material .
	manualset3
145330	5	409331	5	NULL	NULL	0	NULL	multimedia material	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The course was web-based and included synchronous and asynchronous communication , on-line libraries and multimedia material .
	manualset3
145331	1	409332	5	NULL	NULL	0	NULL	creation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The creation of will within the community for CVD research may require additional strategies than in the majority community , such as community organization and local policy development .
	manualset3
145332	2	409332	5	NULL	NULL	0	NULL	will 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The creation of will within the community for CVD research may require additional strategies than in the majority community , such as community organization and local policy development .
	manualset3
145333	3	409332	5	NULL	NULL	0	NULL	community 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The creation of will within the community for CVD research may require additional strategies than in the majority community , such as community organization and local policy development .
	manualset3
145334	4	409332	5	NULL	NULL	0	NULL	CVD research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The creation of will within the community for CVD research may require additional strategies than in the majority community , such as community organization and local policy development .
	manualset3
145335	5	409332	5	NULL	NULL	0	NULL	additional strategies	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The creation of will within the community for CVD research may require additional strategies than in the majority community , such as community organization and local policy development .
	manualset3
145336	6	409332	5	NULL	NULL	0	NULL	majority community 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The creation of will within the community for CVD research may require additional strategies than in the majority community , such as community organization and local policy development .
	manualset3
145337	7	409332	5	NULL	NULL	0	NULL	community organization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The creation of will within the community for CVD research may require additional strategies than in the majority community , such as community organization and local policy development .
	manualset3
145338	8	409332	5	NULL	NULL	0	NULL	local policy development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The creation of will within the community for CVD research may require additional strategies than in the majority community , such as community organization and local policy development .
	manualset3
145339	1	409333	5	NULL	NULL	0	NULL	crimes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The crimes for which clients were arrested tended to be minor : 21 % were for probation or parole violations not associated with new criminal acts , 39 % were for misdemeanors , 27 % were nonviolent felonies , and 12 % were for felonies against persons .
	manualset3
145340	2	409333	5	NULL	NULL	0	NULL	clients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The crimes for which clients were arrested tended to be minor : 21 % were for probation or parole violations not associated with new criminal acts , 39 % were for misdemeanors , 27 % were nonviolent felonies , and 12 % were for felonies against persons .
	manualset3
145341	3	409333	5	NULL	NULL	0	NULL	minor 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The crimes for which clients were arrested tended to be minor : 21 % were for probation or parole violations not associated with new criminal acts , 39 % were for misdemeanors , 27 % were nonviolent felonies , and 12 % were for felonies against persons .
	manualset3
145342	4	409333	5	NULL	NULL	0	NULL	21 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The crimes for which clients were arrested tended to be minor : 21 % were for probation or parole violations not associated with new criminal acts , 39 % were for misdemeanors , 27 % were nonviolent felonies , and 12 % were for felonies against persons .
	manualset3
145343	5	409333	5	NULL	NULL	0	NULL	probation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The crimes for which clients were arrested tended to be minor : 21 % were for probation or parole violations not associated with new criminal acts , 39 % were for misdemeanors , 27 % were nonviolent felonies , and 12 % were for felonies against persons .
	manualset3
145344	6	409333	5	NULL	NULL	0	NULL	parole violations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The crimes for which clients were arrested tended to be minor : 21 % were for probation or parole violations not associated with new criminal acts , 39 % were for misdemeanors , 27 % were nonviolent felonies , and 12 % were for felonies against persons .
	manualset3
145345	7	409333	5	NULL	NULL	0	NULL	criminal acts	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The crimes for which clients were arrested tended to be minor : 21 % were for probation or parole violations not associated with new criminal acts , 39 % were for misdemeanors , 27 % were nonviolent felonies , and 12 % were for felonies against persons .
	manualset3
145346	8	409333	5	NULL	NULL	0	NULL	39 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The crimes for which clients were arrested tended to be minor : 21 % were for probation or parole violations not associated with new criminal acts , 39 % were for misdemeanors , 27 % were nonviolent felonies , and 12 % were for felonies against persons .
	manualset3
145347	9	409333	5	NULL	NULL	0	NULL	misdemeanors 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The crimes for which clients were arrested tended to be minor : 21 % were for probation or parole violations not associated with new criminal acts , 39 % were for misdemeanors , 27 % were nonviolent felonies , and 12 % were for felonies against persons .
	manualset3
145348	10	409333	5	NULL	NULL	0	NULL	27 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The crimes for which clients were arrested tended to be minor : 21 % were for probation or parole violations not associated with new criminal acts , 39 % were for misdemeanors , 27 % were nonviolent felonies , and 12 % were for felonies against persons .
	manualset3
145349	11	409333	5	NULL	NULL	0	NULL	nonviolent felonies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The crimes for which clients were arrested tended to be minor : 21 % were for probation or parole violations not associated with new criminal acts , 39 % were for misdemeanors , 27 % were nonviolent felonies , and 12 % were for felonies against persons .
	manualset3
145350	12	409333	5	NULL	NULL	0	NULL	 12 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The crimes for which clients were arrested tended to be minor : 21 % were for probation or parole violations not associated with new criminal acts , 39 % were for misdemeanors , 27 % were nonviolent felonies , and 12 % were for felonies against persons .
	manualset3
145351	13	409333	5	NULL	NULL	0	NULL	felonies 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The crimes for which clients were arrested tended to be minor : 21 % were for probation or parole violations not associated with new criminal acts , 39 % were for misdemeanors , 27 % were nonviolent felonies , and 12 % were for felonies against persons .
	manualset3
145352	14	409333	5	NULL	NULL	0	NULL	persons 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The crimes for which clients were arrested tended to be minor : 21 % were for probation or parole violations not associated with new criminal acts , 39 % were for misdemeanors , 27 % were nonviolent felonies , and 12 % were for felonies against persons .
	manualset3
145353	1	409334	5	NULL	NULL	0	NULL	association 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3 ) There was an association between physical fitness and whether the break point of respiratory rate was detectable , and the more fit the subject ( above average ) , the more likely the break point was to be undetected .
	manualset3
145354	2	409334	5	NULL	NULL	0	NULL	physical fitness 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3 ) There was an association between physical fitness and whether the break point of respiratory rate was detectable , and the more fit the subject ( above average ) , the more likely the break point was to be undetected .
	manualset3
145355	3	409334	5	NULL	NULL	0	NULL	break point 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3 ) There was an association between physical fitness and whether the break point of respiratory rate was detectable , and the more fit the subject ( above average ) , the more likely the break point was to be undetected .
	manualset3
145356	4	409334	5	NULL	NULL	0	NULL	respiratory rate 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3 ) There was an association between physical fitness and whether the break point of respiratory rate was detectable , and the more fit the subject ( above average ) , the more likely the break point was to be undetected .
	manualset3
145357	5	409334	5	NULL	NULL	0	NULL	subject 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3 ) There was an association between physical fitness and whether the break point of respiratory rate was detectable , and the more fit the subject ( above average ) , the more likely the break point was to be undetected .
	manualset3
145358	6	409334	5	NULL	NULL	0	NULL	above average 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3 ) There was an association between physical fitness and whether the break point of respiratory rate was detectable , and the more fit the subject ( above average ) , the more likely the break point was to be undetected .
	manualset3
145359	7	409334	5	NULL	NULL	0	NULL	break point	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3 ) There was an association between physical fitness and whether the break point of respiratory rate was detectable , and the more fit the subject ( above average ) , the more likely the break point was to be undetected .
	manualset3
145360	1	409335	5	NULL	NULL	0	NULL	criteria 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The criteria for literature selection were that each patient had a history of allergic reaction to local application of ophthalmic drugs or contact lens solutions , and tested positive to putative allergen patch tests .
	manualset3
145361	2	409335	5	NULL	NULL	0	NULL	literature selection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The criteria for literature selection were that each patient had a history of allergic reaction to local application of ophthalmic drugs or contact lens solutions , and tested positive to putative allergen patch tests .
	manualset3
145362	3	409335	5	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The criteria for literature selection were that each patient had a history of allergic reaction to local application of ophthalmic drugs or contact lens solutions , and tested positive to putative allergen patch tests .
	manualset3
145363	4	409335	5	NULL	NULL	0	NULL	history 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The criteria for literature selection were that each patient had a history of allergic reaction to local application of ophthalmic drugs or contact lens solutions , and tested positive to putative allergen patch tests .
	manualset3
145364	5	409335	5	NULL	NULL	0	NULL	allergic reaction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The criteria for literature selection were that each patient had a history of allergic reaction to local application of ophthalmic drugs or contact lens solutions , and tested positive to putative allergen patch tests .
	manualset3
145365	6	409335	5	NULL	NULL	0	NULL	local application	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The criteria for literature selection were that each patient had a history of allergic reaction to local application of ophthalmic drugs or contact lens solutions , and tested positive to putative allergen patch tests .
	manualset3
145366	7	409335	5	NULL	NULL	0	NULL	ophthalmic drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The criteria for literature selection were that each patient had a history of allergic reaction to local application of ophthalmic drugs or contact lens solutions , and tested positive to putative allergen patch tests .
	manualset3
145367	8	409335	5	NULL	NULL	0	NULL	contact lens solutions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The criteria for literature selection were that each patient had a history of allergic reaction to local application of ophthalmic drugs or contact lens solutions , and tested positive to putative allergen patch tests .
	manualset3
145368	9	409335	5	NULL	NULL	0	NULL	putative allergen patch tests	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The criteria for literature selection were that each patient had a history of allergic reaction to local application of ophthalmic drugs or contact lens solutions , and tested positive to putative allergen patch tests .
	manualset3
145369	1	409336	5	NULL	NULL	0	NULL	cross-link density	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cross-link density of the polymer is varied by altering the St/DVB molar ratio .
	manualset3
145370	2	409336	5	NULL	NULL	0	NULL	polymer 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The cross-link density of the polymer is varied by altering the St/DVB molar ratio .
	manualset3
145371	3	409336	5	NULL	NULL	0	NULL	St/DVB molar ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cross-link density of the polymer is varied by altering the St/DVB molar ratio .
	manualset3
145372	1	409337	5	NULL	NULL	0	NULL	cross-resistance	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cross-resistance to topoisomerase II inhibitors occurred earlier than the collateral sensitivity to camptothecin .
	manualset3
145373	2	409337	5	NULL	NULL	0	NULL	topoisomerase II inhibitors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cross-resistance to topoisomerase II inhibitors occurred earlier than the collateral sensitivity to camptothecin .
	manualset3
145374	3	409337	5	NULL	NULL	0	NULL	collateral sensitivity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cross-resistance to topoisomerase II inhibitors occurred earlier than the collateral sensitivity to camptothecin .
	manualset3
145375	4	409337	5	NULL	NULL	0	NULL	camptothecin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The cross-resistance to topoisomerase II inhibitors occurred earlier than the collateral sensitivity to camptothecin .
	manualset3
145376	1	409338	5	NULL	NULL	0	NULL	cross-sectional area reductions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cross-sectional area reductions in combination with ITP allowed visualization of lower concentrations of fluorescently labeled cTnI .
	manualset3
145377	2	409338	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cross-sectional area reductions in combination with ITP allowed visualization of lower concentrations of fluorescently labeled cTnI .
	manualset3
145378	3	409338	5	NULL	NULL	NULL	NULL	ITP 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The cross-sectional area reductions in combination with ITP allowed visualization of lower concentrations of fluorescently labeled cTnI .
	manualset3
145379	4	409338	5	NULL	NULL	0	NULL	visualization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cross-sectional area reductions in combination with ITP allowed visualization of lower concentrations of fluorescently labeled cTnI .
	manualset3
145380	5	409338	5	NULL	NULL	0	NULL	concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cross-sectional area reductions in combination with ITP allowed visualization of lower concentrations of fluorescently labeled cTnI .
	manualset3
145381	6	409338	5	NULL	NULL	0	NULL	fluorescently labeled cTnI	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The cross-sectional area reductions in combination with ITP allowed visualization of lower concentrations of fluorescently labeled cTnI .
	manualset3
145382	1	409339	5	NULL	NULL	0	NULL	crosslinking reactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The crosslinking reactions were characterized by ( 1 ) H NMR and IR spectroscopies , differential scanning calorimetry ( DSC ) , and dynamic light scattering ( DLS ) measurements .
	manualset3
145383	2	409339	5	NULL	NULL	0	NULL	H NMR spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The crosslinking reactions were characterized by ( 1 ) H NMR and IR spectroscopies , differential scanning calorimetry ( DSC ) , and dynamic light scattering ( DLS ) measurements .
	manualset3
145384	3	409339	5	NULL	NULL	0	NULL	IR spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The crosslinking reactions were characterized by ( 1 ) H NMR and IR spectroscopies , differential scanning calorimetry ( DSC ) , and dynamic light scattering ( DLS ) measurements .
	manualset3
145385	4	409339	5	NULL	NULL	0	NULL	differential scanning calorimetry ( DSC )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The crosslinking reactions were characterized by ( 1 ) H NMR and IR spectroscopies , differential scanning calorimetry ( DSC ) , and dynamic light scattering ( DLS ) measurements .
	manualset3
145386	5	409339	5	NULL	NULL	0	NULL	dynamic light scattering ( DLS ) measurements	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The crosslinking reactions were characterized by ( 1 ) H NMR and IR spectroscopies , differential scanning calorimetry ( DSC ) , and dynamic light scattering ( DLS ) measurements .
	manualset3
145387	1	409340	5	NULL	NULL	0	NULL	crude protein content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The crude protein content of the three forages was 4.9 , 9.4 , and 12.2 % for low - , medium - , and high-quality forages , respectively .
	manualset3
145388	2	409340	5	NULL	NULL	0	NULL	three 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The crude protein content of the three forages was 4.9 , 9.4 , and 12.2 % for low - , medium - , and high-quality forages , respectively .
	manualset3
145389	3	409340	5	NULL	NULL	0	NULL	forages 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The crude protein content of the three forages was 4.9 , 9.4 , and 12.2 % for low - , medium - , and high-quality forages , respectively .
	manualset3
145390	4	409340	5	NULL	NULL	0	NULL	 4.9%	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The crude protein content of the three forages was 4.9 , 9.4 , and 12.2 % for low - , medium - , and high-quality forages , respectively .
	manualset3
145391	5	409340	5	NULL	NULL	0	NULL	9.4 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The crude protein content of the three forages was 4.9 , 9.4 , and 12.2 % for low - , medium - , and high-quality forages , respectively .
	manualset3
145392	6	409340	5	NULL	NULL	0	NULL	12.2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The crude protein content of the three forages was 4.9 , 9.4 , and 12.2 % for low - , medium - , and high-quality forages , respectively .
	manualset3
145393	7	409340	5	NULL	NULL	0	NULL	low-quality forages	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The crude protein content of the three forages was 4.9 , 9.4 , and 12.2 % for low - , medium - , and high-quality forages , respectively .
	manualset3
145394	8	409340	5	NULL	NULL	0	NULL	medium-quality forages	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The crude protein content of the three forages was 4.9 , 9.4 , and 12.2 % for low - , medium - , and high-quality forages , respectively .
	manualset3
145395	9	409340	5	NULL	NULL	0	NULL	high-quality forages	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The crude protein content of the three forages was 4.9 , 9.4 , and 12.2 % for low - , medium - , and high-quality forages , respectively .
	manualset3
145396	1	409341	5	NULL	NULL	0	NULL	crude venom	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The crude venom of many elapid snakes appeared to contain proteins that activated blood coagulation factor V. The factor V activator present in the venom of Naja naja oxiana was purified to homogeneity by chromatography on a mono-S column .
	manualset3
145397	2	409341	5	NULL	NULL	0	NULL	elapid snakes 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The crude venom of many elapid snakes appeared to contain proteins that activated blood coagulation factor V. The factor V activator present in the venom of Naja naja oxiana was purified to homogeneity by chromatography on a mono-S column .
	manualset3
145398	3	409341	5	NULL	NULL	0	NULL	proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The crude venom of many elapid snakes appeared to contain proteins that activated blood coagulation factor V. The factor V activator present in the venom of Naja naja oxiana was purified to homogeneity by chromatography on a mono-S column .
	manualset3
145399	4	409341	5	NULL	NULL	0	NULL	blood coagulation factor V	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The crude venom of many elapid snakes appeared to contain proteins that activated blood coagulation factor V. The factor V activator present in the venom of Naja naja oxiana was purified to homogeneity by chromatography on a mono-S column .
	manualset3
145400	5	409341	5	NULL	NULL	0	NULL	factor V activator	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The crude venom of many elapid snakes appeared to contain proteins that activated blood coagulation factor V. The factor V activator present in the venom of Naja naja oxiana was purified to homogeneity by chromatography on a mono-S column .
	manualset3
145401	6	409341	5	NULL	NULL	0	NULL	venom 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The crude venom of many elapid snakes appeared to contain proteins that activated blood coagulation factor V. The factor V activator present in the venom of Naja naja oxiana was purified to homogeneity by chromatography on a mono-S column .
	manualset3
145402	7	409341	5	NULL	NULL	0	NULL	Naja naja oxiana	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The crude venom of many elapid snakes appeared to contain proteins that activated blood coagulation factor V. The factor V activator present in the venom of Naja naja oxiana was purified to homogeneity by chromatography on a mono-S column .
	manualset3
145403	8	409341	5	NULL	NULL	0	NULL	homogeneity 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The crude venom of many elapid snakes appeared to contain proteins that activated blood coagulation factor V. The factor V activator present in the venom of Naja naja oxiana was purified to homogeneity by chromatography on a mono-S column .
	manualset3
145404	9	409341	5	NULL	NULL	0	NULL	chromatography 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The crude venom of many elapid snakes appeared to contain proteins that activated blood coagulation factor V. The factor V activator present in the venom of Naja naja oxiana was purified to homogeneity by chromatography on a mono-S column .
	manualset3
145405	10	409341	5	NULL	NULL	0	NULL	mono-S column	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The crude venom of many elapid snakes appeared to contain proteins that activated blood coagulation factor V. The factor V activator present in the venom of Naja naja oxiana was purified to homogeneity by chromatography on a mono-S column .
	manualset3
145406	1	409342	5	NULL	NULL	0	NULL	pattern 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar pattern was observed in the pre-treated group 4 h after the administration of paracetamol with a reduction in serum levels of ALT , aspartate aminotransferase and alkaline phosphatase enzymes by 65.04 , 55.79 and 45.75 % respectively ( P & lt ; 0.001 ) .
	manualset3
145407	2	409342	5	NULL	NULL	0	NULL	pre-treated group 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar pattern was observed in the pre-treated group 4 h after the administration of paracetamol with a reduction in serum levels of ALT , aspartate aminotransferase and alkaline phosphatase enzymes by 65.04 , 55.79 and 45.75 % respectively ( P & lt ; 0.001 ) .
	manualset3
145408	3	409342	5	NULL	NULL	0	NULL	4 h 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar pattern was observed in the pre-treated group 4 h after the administration of paracetamol with a reduction in serum levels of ALT , aspartate aminotransferase and alkaline phosphatase enzymes by 65.04 , 55.79 and 45.75 % respectively ( P & lt ; 0.001 ) .
	manualset3
145409	4	409342	5	NULL	NULL	0	NULL	administration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar pattern was observed in the pre-treated group 4 h after the administration of paracetamol with a reduction in serum levels of ALT , aspartate aminotransferase and alkaline phosphatase enzymes by 65.04 , 55.79 and 45.75 % respectively ( P & lt ; 0.001 ) .
	manualset3
145410	5	409342	5	NULL	NULL	0	NULL	paracetamol 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar pattern was observed in the pre-treated group 4 h after the administration of paracetamol with a reduction in serum levels of ALT , aspartate aminotransferase and alkaline phosphatase enzymes by 65.04 , 55.79 and 45.75 % respectively ( P & lt ; 0.001 ) .
	manualset3
145411	6	409342	5	NULL	NULL	0	NULL	reduction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar pattern was observed in the pre-treated group 4 h after the administration of paracetamol with a reduction in serum levels of ALT , aspartate aminotransferase and alkaline phosphatase enzymes by 65.04 , 55.79 and 45.75 % respectively ( P & lt ; 0.001 ) .
	manualset3
145412	7	409342	5	NULL	NULL	0	NULL	serum levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar pattern was observed in the pre-treated group 4 h after the administration of paracetamol with a reduction in serum levels of ALT , aspartate aminotransferase and alkaline phosphatase enzymes by 65.04 , 55.79 and 45.75 % respectively ( P & lt ; 0.001 ) .
	manualset3
145413	8	409342	5	NULL	NULL	0	NULL	ALT 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar pattern was observed in the pre-treated group 4 h after the administration of paracetamol with a reduction in serum levels of ALT , aspartate aminotransferase and alkaline phosphatase enzymes by 65.04 , 55.79 and 45.75 % respectively ( P & lt ; 0.001 ) .
	manualset3
145414	9	409342	5	NULL	NULL	0	NULL	aspartate aminotransferase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar pattern was observed in the pre-treated group 4 h after the administration of paracetamol with a reduction in serum levels of ALT , aspartate aminotransferase and alkaline phosphatase enzymes by 65.04 , 55.79 and 45.75 % respectively ( P & lt ; 0.001 ) .
	manualset3
145415	10	409342	5	NULL	NULL	0	NULL	alkaline phosphatase enzymes	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar pattern was observed in the pre-treated group 4 h after the administration of paracetamol with a reduction in serum levels of ALT , aspartate aminotransferase and alkaline phosphatase enzymes by 65.04 , 55.79 and 45.75 % respectively ( P & lt ; 0.001 ) .
	manualset3
145416	11	409342	5	NULL	NULL	0	NULL	65.04 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar pattern was observed in the pre-treated group 4 h after the administration of paracetamol with a reduction in serum levels of ALT , aspartate aminotransferase and alkaline phosphatase enzymes by 65.04 , 55.79 and 45.75 % respectively ( P & lt ; 0.001 ) .
	manualset3
145417	12	409342	5	NULL	NULL	0	NULL	55.79 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar pattern was observed in the pre-treated group 4 h after the administration of paracetamol with a reduction in serum levels of ALT , aspartate aminotransferase and alkaline phosphatase enzymes by 65.04 , 55.79 and 45.75 % respectively ( P & lt ; 0.001 ) .
	manualset3
145418	13	409342	5	NULL	NULL	0	NULL	45.75 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar pattern was observed in the pre-treated group 4 h after the administration of paracetamol with a reduction in serum levels of ALT , aspartate aminotransferase and alkaline phosphatase enzymes by 65.04 , 55.79 and 45.75 % respectively ( P & lt ; 0.001 ) .
	manualset3
145419	14	409342	5	NULL	NULL	0	NULL	 P & lt ; 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar pattern was observed in the pre-treated group 4 h after the administration of paracetamol with a reduction in serum levels of ALT , aspartate aminotransferase and alkaline phosphatase enzymes by 65.04 , 55.79 and 45.75 % respectively ( P & lt ; 0.001 ) .
	manualset3
145420	1	409343	5	NULL	NULL	0	NULL	crustacean isopod Armadillidium vulgare 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The crustacean isopod Armadillidium vulgare is characterized by an unusual approximately 42-kb-long mitochondrial genome consisting of two molecules co-occurring in mitochondria : a circular approximately 28-kb dimer formed by two approximately 14-kb monomers fused in opposite polarities and a linear approximately 14-kb monomer .
	manualset3
145421	2	409343	5	NULL	NULL	0	NULL	42-kb-long mitochondrial genome 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The crustacean isopod Armadillidium vulgare is characterized by an unusual approximately 42-kb-long mitochondrial genome consisting of two molecules co-occurring in mitochondria : a circular approximately 28-kb dimer formed by two approximately 14-kb monomers fused in opposite polarities and a linear approximately 14-kb monomer .
	manualset3
145422	3	409343	5	NULL	NULL	0	NULL	two molecules 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The crustacean isopod Armadillidium vulgare is characterized by an unusual approximately 42-kb-long mitochondrial genome consisting of two molecules co-occurring in mitochondria : a circular approximately 28-kb dimer formed by two approximately 14-kb monomers fused in opposite polarities and a linear approximately 14-kb monomer .
	manualset3
145423	4	409343	5	NULL	NULL	0	NULL	mitochondria 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The crustacean isopod Armadillidium vulgare is characterized by an unusual approximately 42-kb-long mitochondrial genome consisting of two molecules co-occurring in mitochondria : a circular approximately 28-kb dimer formed by two approximately 14-kb monomers fused in opposite polarities and a linear approximately 14-kb monomer .
	manualset3
145424	5	409343	5	NULL	NULL	0	NULL	28-kb dimer	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The crustacean isopod Armadillidium vulgare is characterized by an unusual approximately 42-kb-long mitochondrial genome consisting of two molecules co-occurring in mitochondria : a circular approximately 28-kb dimer formed by two approximately 14-kb monomers fused in opposite polarities and a linear approximately 14-kb monomer .
	manualset3
145425	6	409343	5	NULL	NULL	NULL	NULL	two	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The crustacean isopod Armadillidium vulgare is characterized by an unusual approximately 42-kb-long mitochondrial genome consisting of two molecules co-occurring in mitochondria : a circular approximately 28-kb dimer formed by two approximately 14-kb monomers fused in opposite polarities and a linear approximately 14-kb monomer .
	manualset3
145426	7	409343	5	NULL	NULL	0	NULL	14-kb monomers	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The crustacean isopod Armadillidium vulgare is characterized by an unusual approximately 42-kb-long mitochondrial genome consisting of two molecules co-occurring in mitochondria : a circular approximately 28-kb dimer formed by two approximately 14-kb monomers fused in opposite polarities and a linear approximately 14-kb monomer .
	manualset3
145427	8	409343	5	NULL	NULL	0	NULL	opposite polarities 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The crustacean isopod Armadillidium vulgare is characterized by an unusual approximately 42-kb-long mitochondrial genome consisting of two molecules co-occurring in mitochondria : a circular approximately 28-kb dimer formed by two approximately 14-kb monomers fused in opposite polarities and a linear approximately 14-kb monomer .
	manualset3
145428	9	409343	5	NULL	NULL	0	NULL	14-kb monomer 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The crustacean isopod Armadillidium vulgare is characterized by an unusual approximately 42-kb-long mitochondrial genome consisting of two molecules co-occurring in mitochondria : a circular approximately 28-kb dimer formed by two approximately 14-kb monomers fused in opposite polarities and a linear approximately 14-kb monomer .
	manualset3
145429	1	409344	5	NULL	NULL	0	NULL	crystal structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure is stabilized by O-HN hydrogen bonds .
	manualset3
145430	2	409344	5	NULL	NULL	0	NULL	O-HN hydrogen bonds	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure is stabilized by O-HN hydrogen bonds .
	manualset3
145431	1	409345	5	NULL	NULL	0	NULL	crystal structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of ( Pu ( 4 ) ( NO ( 3 ) ) ( 8 ) ( HdCMP ) ( 4 ) ( H ( 2 ) O ) ( 8 ) ) ( NO ( 3 ) ) ( 4 ) .2 H ( 2 ) O consists of complex cations ( Pu ( 4 ) ( NO ( 3 ) ) ( 8 ) ( HdCMP ) ( 4 ) ( H ( 2 ) O ) ( 8 ) ) ( 4 + ) , NO ( 3 ) ( - ) anions , and water molecules .
	manualset3
145432	2	409345	5	NULL	NULL	0	NULL	( Pu ( 4 ) ( NO ( 3 ) ) ( 8 ) ( HdCMP ) ( 4 ) ( H ( 2 ) O ) ( 8 ) ) ( NO ( 3 ) ) ( 4 ) .2 H ( 2 ) O 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of ( Pu ( 4 ) ( NO ( 3 ) ) ( 8 ) ( HdCMP ) ( 4 ) ( H ( 2 ) O ) ( 8 ) ) ( NO ( 3 ) ) ( 4 ) .2 H ( 2 ) O consists of complex cations ( Pu ( 4 ) ( NO ( 3 ) ) ( 8 ) ( HdCMP ) ( 4 ) ( H ( 2 ) O ) ( 8 ) ) ( 4 + ) , NO ( 3 ) ( - ) anions , and water molecules .
	manualset3
145433	3	409345	5	NULL	NULL	0	NULL	complex cations	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of ( Pu ( 4 ) ( NO ( 3 ) ) ( 8 ) ( HdCMP ) ( 4 ) ( H ( 2 ) O ) ( 8 ) ) ( NO ( 3 ) ) ( 4 ) .2 H ( 2 ) O consists of complex cations ( Pu ( 4 ) ( NO ( 3 ) ) ( 8 ) ( HdCMP ) ( 4 ) ( H ( 2 ) O ) ( 8 ) ) ( 4 + ) , NO ( 3 ) ( - ) anions , and water molecules .
	manualset3
145434	4	409345	5	NULL	NULL	0	NULL	( Pu ( 4 ) ( NO ( 3 ) ) ( 8 ) ( HdCMP ) ( 4 ) ( H ( 2 ) O ) ( 8 ) ) ( 4 + ) , NO ( 3 ) ( - ) anions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of ( Pu ( 4 ) ( NO ( 3 ) ) ( 8 ) ( HdCMP ) ( 4 ) ( H ( 2 ) O ) ( 8 ) ) ( NO ( 3 ) ) ( 4 ) .2 H ( 2 ) O consists of complex cations ( Pu ( 4 ) ( NO ( 3 ) ) ( 8 ) ( HdCMP ) ( 4 ) ( H ( 2 ) O ) ( 8 ) ) ( 4 + ) , NO ( 3 ) ( - ) anions , and water molecules .
	manualset3
145435	5	409345	5	NULL	NULL	0	NULL	water molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of ( Pu ( 4 ) ( NO ( 3 ) ) ( 8 ) ( HdCMP ) ( 4 ) ( H ( 2 ) O ) ( 8 ) ) ( NO ( 3 ) ) ( 4 ) .2 H ( 2 ) O consists of complex cations ( Pu ( 4 ) ( NO ( 3 ) ) ( 8 ) ( HdCMP ) ( 4 ) ( H ( 2 ) O ) ( 8 ) ) ( 4 + ) , NO ( 3 ) ( - ) anions , and water molecules .
	manualset3
145436	1	409346	5	NULL	NULL	0	NULL	crystal structure 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of D-lactate dehydrogenase from Aquifex aeolicus ( aq_727 ) was determined to 2.12 A resolution in space group P2 ( 1 ) 2 ( 1 ) 2 ( 1 ) , with unit-cell parameters a = 90.94 , b = 94.43 , c = 188.85 A. The structure was solved by molecular replacement using the coenzyme-binding domain of Lactobacillus helveticus D-lactate dehydrogenase and contained two homodimers in the asymmetric unit .
	manualset3
145437	2	409346	5	NULL	NULL	0	NULL	D-lactate dehydrogenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of D-lactate dehydrogenase from Aquifex aeolicus ( aq_727 ) was determined to 2.12 A resolution in space group P2 ( 1 ) 2 ( 1 ) 2 ( 1 ) , with unit-cell parameters a = 90.94 , b = 94.43 , c = 188.85 A. The structure was solved by molecular replacement using the coenzyme-binding domain of Lactobacillus helveticus D-lactate dehydrogenase and contained two homodimers in the asymmetric unit .
	manualset3
145438	3	409346	5	NULL	NULL	0	NULL	Aquifex aeolicus ( aq_727 )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of D-lactate dehydrogenase from Aquifex aeolicus ( aq_727 ) was determined to 2.12 A resolution in space group P2 ( 1 ) 2 ( 1 ) 2 ( 1 ) , with unit-cell parameters a = 90.94 , b = 94.43 , c = 188.85 A. The structure was solved by molecular replacement using the coenzyme-binding domain of Lactobacillus helveticus D-lactate dehydrogenase and contained two homodimers in the asymmetric unit .
	manualset3
145439	4	409346	5	NULL	NULL	0	NULL	2.12 A resolution	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of D-lactate dehydrogenase from Aquifex aeolicus ( aq_727 ) was determined to 2.12 A resolution in space group P2 ( 1 ) 2 ( 1 ) 2 ( 1 ) , with unit-cell parameters a = 90.94 , b = 94.43 , c = 188.85 A. The structure was solved by molecular replacement using the coenzyme-binding domain of Lactobacillus helveticus D-lactate dehydrogenase and contained two homodimers in the asymmetric unit .
	manualset3
145440	5	409346	5	NULL	NULL	0	NULL	space group P2 ( 1 ) 2 ( 1 ) 2 ( 1 ) 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of D-lactate dehydrogenase from Aquifex aeolicus ( aq_727 ) was determined to 2.12 A resolution in space group P2 ( 1 ) 2 ( 1 ) 2 ( 1 ) , with unit-cell parameters a = 90.94 , b = 94.43 , c = 188.85 A. The structure was solved by molecular replacement using the coenzyme-binding domain of Lactobacillus helveticus D-lactate dehydrogenase and contained two homodimers in the asymmetric unit .
	manualset3
145441	6	409346	5	NULL	NULL	0	NULL	unit-cell parameters	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of D-lactate dehydrogenase from Aquifex aeolicus ( aq_727 ) was determined to 2.12 A resolution in space group P2 ( 1 ) 2 ( 1 ) 2 ( 1 ) , with unit-cell parameters a = 90.94 , b = 94.43 , c = 188.85 A. The structure was solved by molecular replacement using the coenzyme-binding domain of Lactobacillus helveticus D-lactate dehydrogenase and contained two homodimers in the asymmetric unit .
	manualset3
145442	7	409346	5	NULL	NULL	0	NULL	a = 90.94	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of D-lactate dehydrogenase from Aquifex aeolicus ( aq_727 ) was determined to 2.12 A resolution in space group P2 ( 1 ) 2 ( 1 ) 2 ( 1 ) , with unit-cell parameters a = 90.94 , b = 94.43 , c = 188.85 A. The structure was solved by molecular replacement using the coenzyme-binding domain of Lactobacillus helveticus D-lactate dehydrogenase and contained two homodimers in the asymmetric unit .
	manualset3
145443	8	409346	5	NULL	NULL	0	NULL	b = 94.43	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of D-lactate dehydrogenase from Aquifex aeolicus ( aq_727 ) was determined to 2.12 A resolution in space group P2 ( 1 ) 2 ( 1 ) 2 ( 1 ) , with unit-cell parameters a = 90.94 , b = 94.43 , c = 188.85 A. The structure was solved by molecular replacement using the coenzyme-binding domain of Lactobacillus helveticus D-lactate dehydrogenase and contained two homodimers in the asymmetric unit .
	manualset3
145444	9	409346	5	NULL	NULL	0	NULL	c = 188.85 A	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of D-lactate dehydrogenase from Aquifex aeolicus ( aq_727 ) was determined to 2.12 A resolution in space group P2 ( 1 ) 2 ( 1 ) 2 ( 1 ) , with unit-cell parameters a = 90.94 , b = 94.43 , c = 188.85 A. The structure was solved by molecular replacement using the coenzyme-binding domain of Lactobacillus helveticus D-lactate dehydrogenase and contained two homodimers in the asymmetric unit .
	manualset3
145445	10	409346	5	NULL	NULL	0	NULL	structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of D-lactate dehydrogenase from Aquifex aeolicus ( aq_727 ) was determined to 2.12 A resolution in space group P2 ( 1 ) 2 ( 1 ) 2 ( 1 ) , with unit-cell parameters a = 90.94 , b = 94.43 , c = 188.85 A. The structure was solved by molecular replacement using the coenzyme-binding domain of Lactobacillus helveticus D-lactate dehydrogenase and contained two homodimers in the asymmetric unit .
	manualset3
145446	11	409346	5	NULL	NULL	0	NULL	molecular replacement	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of D-lactate dehydrogenase from Aquifex aeolicus ( aq_727 ) was determined to 2.12 A resolution in space group P2 ( 1 ) 2 ( 1 ) 2 ( 1 ) , with unit-cell parameters a = 90.94 , b = 94.43 , c = 188.85 A. The structure was solved by molecular replacement using the coenzyme-binding domain of Lactobacillus helveticus D-lactate dehydrogenase and contained two homodimers in the asymmetric unit .
	manualset3
145447	12	409346	5	NULL	NULL	0	NULL	coenzyme-binding domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of D-lactate dehydrogenase from Aquifex aeolicus ( aq_727 ) was determined to 2.12 A resolution in space group P2 ( 1 ) 2 ( 1 ) 2 ( 1 ) , with unit-cell parameters a = 90.94 , b = 94.43 , c = 188.85 A. The structure was solved by molecular replacement using the coenzyme-binding domain of Lactobacillus helveticus D-lactate dehydrogenase and contained two homodimers in the asymmetric unit .
	manualset3
145448	13	409346	5	NULL	NULL	0	NULL	Lactobacillus helveticus D-lactate dehydrogenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of D-lactate dehydrogenase from Aquifex aeolicus ( aq_727 ) was determined to 2.12 A resolution in space group P2 ( 1 ) 2 ( 1 ) 2 ( 1 ) , with unit-cell parameters a = 90.94 , b = 94.43 , c = 188.85 A. The structure was solved by molecular replacement using the coenzyme-binding domain of Lactobacillus helveticus D-lactate dehydrogenase and contained two homodimers in the asymmetric unit .
	manualset3
145449	14	409346	5	NULL	NULL	0	NULL	two homodimers	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of D-lactate dehydrogenase from Aquifex aeolicus ( aq_727 ) was determined to 2.12 A resolution in space group P2 ( 1 ) 2 ( 1 ) 2 ( 1 ) , with unit-cell parameters a = 90.94 , b = 94.43 , c = 188.85 A. The structure was solved by molecular replacement using the coenzyme-binding domain of Lactobacillus helveticus D-lactate dehydrogenase and contained two homodimers in the asymmetric unit .
	manualset3
145450	15	409346	5	NULL	NULL	0	NULL	asymmetric unit 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of D-lactate dehydrogenase from Aquifex aeolicus ( aq_727 ) was determined to 2.12 A resolution in space group P2 ( 1 ) 2 ( 1 ) 2 ( 1 ) , with unit-cell parameters a = 90.94 , b = 94.43 , c = 188.85 A. The structure was solved by molecular replacement using the coenzyme-binding domain of Lactobacillus helveticus D-lactate dehydrogenase and contained two homodimers in the asymmetric unit .
	manualset3
145451	1	409347	5	NULL	NULL	0	NULL	crystal structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of methyl 6-O-benzyl-2-deoxy-2-dimethylmaleimido -- D-allopyranoside was solved in order to gain insight into the hydrogen bond features which can be determining features in the glycosylation regioselectivity observed for this compound .
	manualset3
145452	2	409347	5	NULL	NULL	0	NULL	methyl 6-O-benzyl-2-deoxy-2-dimethylmaleimido -- D-allopyranoside 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of methyl 6-O-benzyl-2-deoxy-2-dimethylmaleimido -- D-allopyranoside was solved in order to gain insight into the hydrogen bond features which can be determining features in the glycosylation regioselectivity observed for this compound .
	manualset3
145453	3	409347	5	NULL	NULL	0	NULL	insight 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of methyl 6-O-benzyl-2-deoxy-2-dimethylmaleimido -- D-allopyranoside was solved in order to gain insight into the hydrogen bond features which can be determining features in the glycosylation regioselectivity observed for this compound .
	manualset3
145454	4	409347	5	NULL	NULL	0	NULL	hydrogen bond features 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of methyl 6-O-benzyl-2-deoxy-2-dimethylmaleimido -- D-allopyranoside was solved in order to gain insight into the hydrogen bond features which can be determining features in the glycosylation regioselectivity observed for this compound .
	manualset3
145455	5	409347	5	NULL	NULL	0	NULL	determining features 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of methyl 6-O-benzyl-2-deoxy-2-dimethylmaleimido -- D-allopyranoside was solved in order to gain insight into the hydrogen bond features which can be determining features in the glycosylation regioselectivity observed for this compound .
	manualset3
145456	6	409347	5	NULL	NULL	0	NULL	glycosylation regioselectivity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of methyl 6-O-benzyl-2-deoxy-2-dimethylmaleimido -- D-allopyranoside was solved in order to gain insight into the hydrogen bond features which can be determining features in the glycosylation regioselectivity observed for this compound .
	manualset3
145457	7	409347	5	NULL	NULL	0	NULL	compound 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of methyl 6-O-benzyl-2-deoxy-2-dimethylmaleimido -- D-allopyranoside was solved in order to gain insight into the hydrogen bond features which can be determining features in the glycosylation regioselectivity observed for this compound .
	manualset3
145458	1	409348	5	NULL	NULL	0	NULL	crystal structure 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of the AHI-1 SH3 domain thus provides a valuable tool for identification of key interaction sites in regulation of drug resistance and for the development of small molecule inhibitors for CML .
	manualset3
145459	2	409348	5	NULL	NULL	0	NULL	AHI-1 SH3 domain 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of the AHI-1 SH3 domain thus provides a valuable tool for identification of key interaction sites in regulation of drug resistance and for the development of small molecule inhibitors for CML .
	manualset3
145460	3	409348	5	NULL	NULL	0	NULL	 valuable tool 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of the AHI-1 SH3 domain thus provides a valuable tool for identification of key interaction sites in regulation of drug resistance and for the development of small molecule inhibitors for CML .
	manualset3
145461	4	409348	5	NULL	NULL	0	NULL	identification 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of the AHI-1 SH3 domain thus provides a valuable tool for identification of key interaction sites in regulation of drug resistance and for the development of small molecule inhibitors for CML .
	manualset3
145462	5	409348	5	NULL	NULL	0	NULL	interaction sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of the AHI-1 SH3 domain thus provides a valuable tool for identification of key interaction sites in regulation of drug resistance and for the development of small molecule inhibitors for CML .
	manualset3
145463	6	409348	5	NULL	NULL	0	NULL	regulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of the AHI-1 SH3 domain thus provides a valuable tool for identification of key interaction sites in regulation of drug resistance and for the development of small molecule inhibitors for CML .
	manualset3
145464	7	409348	5	NULL	NULL	0	NULL	drug resistance	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of the AHI-1 SH3 domain thus provides a valuable tool for identification of key interaction sites in regulation of drug resistance and for the development of small molecule inhibitors for CML .
	manualset3
145465	8	409348	5	NULL	NULL	0	NULL	development 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of the AHI-1 SH3 domain thus provides a valuable tool for identification of key interaction sites in regulation of drug resistance and for the development of small molecule inhibitors for CML .
	manualset3
145466	9	409348	5	NULL	NULL	0	NULL	small molecule inhibitors	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of the AHI-1 SH3 domain thus provides a valuable tool for identification of key interaction sites in regulation of drug resistance and for the development of small molecule inhibitors for CML .
	manualset3
145467	10	409348	5	NULL	NULL	0	NULL	CML 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystal structure of the AHI-1 SH3 domain thus provides a valuable tool for identification of key interaction sites in regulation of drug resistance and for the development of small molecule inhibitors for CML .
	manualset3
145468	1	409349	5	NULL	NULL	0	NULL	crystals 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystals are hexagonal with a P6 ( 4 ) 22 space group , which differs significantly from that of crystals of the free protein .
	manualset3
145469	2	409349	5	NULL	NULL	0	NULL	P6 ( 4 ) 22 space group 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystals are hexagonal with a P6 ( 4 ) 22 space group , which differs significantly from that of crystals of the free protein .
	manualset3
145470	3	409349	5	NULL	NULL	0	NULL	crystals 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystals are hexagonal with a P6 ( 4 ) 22 space group , which differs significantly from that of crystals of the free protein .
	manualset3
145471	4	409349	5	NULL	NULL	0	NULL	free protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The crystals are hexagonal with a P6 ( 4 ) 22 space group , which differs significantly from that of crystals of the free protein .
	manualset3
145472	1	409350	5	NULL	NULL	0	NULL	cultivars 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The cultivars with colored seed coats contained higher amounts of polyphenols .
	manualset3
145473	2	409350	5	NULL	NULL	0	NULL	colored seed coats	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The cultivars with colored seed coats contained higher amounts of polyphenols .
	manualset3
145474	3	409350	5	NULL	NULL	0	NULL	higher amounts 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cultivars with colored seed coats contained higher amounts of polyphenols .
	manualset3
145475	4	409350	5	NULL	NULL	0	NULL	polyphenols 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The cultivars with colored seed coats contained higher amounts of polyphenols .
	manualset3
145476	1	409351	5	NULL	NULL	0	NULL	percentage 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar percentage of MMTV-MAT/neu and MMTV-neu tumors acquired deletions in the neu transgene , which have previously been shown to result in constitutive receptor activation .
	manualset3
145477	2	409351	5	NULL	NULL	0	NULL	MMTV-MAT/neu 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar percentage of MMTV-MAT/neu and MMTV-neu tumors acquired deletions in the neu transgene , which have previously been shown to result in constitutive receptor activation .
	manualset3
145478	3	409351	5	NULL	NULL	0	NULL	MMTV-neu tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar percentage of MMTV-MAT/neu and MMTV-neu tumors acquired deletions in the neu transgene , which have previously been shown to result in constitutive receptor activation .
	manualset3
145479	4	409351	5	NULL	NULL	0	NULL	deletions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar percentage of MMTV-MAT/neu and MMTV-neu tumors acquired deletions in the neu transgene , which have previously been shown to result in constitutive receptor activation .
	manualset3
145480	5	409351	5	NULL	NULL	0	NULL	neu transgene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar percentage of MMTV-MAT/neu and MMTV-neu tumors acquired deletions in the neu transgene , which have previously been shown to result in constitutive receptor activation .
	manualset3
145481	6	409351	5	NULL	NULL	0	NULL	result 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar percentage of MMTV-MAT/neu and MMTV-neu tumors acquired deletions in the neu transgene , which have previously been shown to result in constitutive receptor activation .
	manualset3
145482	7	409351	5	NULL	NULL	0	NULL	constitutive receptor activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar percentage of MMTV-MAT/neu and MMTV-neu tumors acquired deletions in the neu transgene , which have previously been shown to result in constitutive receptor activation .
	manualset3
145483	1	409352	5	NULL	NULL	0	NULL	culture medium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The culture medium included 10-100 units/ml of recombinant lymphokines ( rIL-1 , rIL-2 , rIL-4 , rIL-6 and rIL-7 ) and 10 % fetal calf serum in RPMI-1640 medium .
	manualset3
145484	2	409352	5	NULL	NULL	0	NULL	10-100 units/ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The culture medium included 10-100 units/ml of recombinant lymphokines ( rIL-1 , rIL-2 , rIL-4 , rIL-6 and rIL-7 ) and 10 % fetal calf serum in RPMI-1640 medium .
	manualset3
145485	3	409352	5	NULL	NULL	0	NULL	recombinant lymphokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The culture medium included 10-100 units/ml of recombinant lymphokines ( rIL-1 , rIL-2 , rIL-4 , rIL-6 and rIL-7 ) and 10 % fetal calf serum in RPMI-1640 medium .
	manualset3
145486	4	409352	5	NULL	NULL	0	NULL	rIL-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The culture medium included 10-100 units/ml of recombinant lymphokines ( rIL-1 , rIL-2 , rIL-4 , rIL-6 and rIL-7 ) and 10 % fetal calf serum in RPMI-1640 medium .
	manualset3
145487	5	409352	5	NULL	NULL	0	NULL	rIL-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The culture medium included 10-100 units/ml of recombinant lymphokines ( rIL-1 , rIL-2 , rIL-4 , rIL-6 and rIL-7 ) and 10 % fetal calf serum in RPMI-1640 medium .
	manualset3
145488	6	409352	5	NULL	NULL	0	NULL	rIL-4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The culture medium included 10-100 units/ml of recombinant lymphokines ( rIL-1 , rIL-2 , rIL-4 , rIL-6 and rIL-7 ) and 10 % fetal calf serum in RPMI-1640 medium .
	manualset3
145489	7	409352	5	NULL	NULL	0	NULL	rIL-6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The culture medium included 10-100 units/ml of recombinant lymphokines ( rIL-1 , rIL-2 , rIL-4 , rIL-6 and rIL-7 ) and 10 % fetal calf serum in RPMI-1640 medium .
	manualset3
145490	8	409352	5	NULL	NULL	0	NULL	rIL-7	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The culture medium included 10-100 units/ml of recombinant lymphokines ( rIL-1 , rIL-2 , rIL-4 , rIL-6 and rIL-7 ) and 10 % fetal calf serum in RPMI-1640 medium .
	manualset3
145491	9	409352	5	NULL	NULL	0	NULL	10 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The culture medium included 10-100 units/ml of recombinant lymphokines ( rIL-1 , rIL-2 , rIL-4 , rIL-6 and rIL-7 ) and 10 % fetal calf serum in RPMI-1640 medium .
	manualset3
145492	10	409352	5	NULL	NULL	0	NULL	fetal calf serum	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The culture medium included 10-100 units/ml of recombinant lymphokines ( rIL-1 , rIL-2 , rIL-4 , rIL-6 and rIL-7 ) and 10 % fetal calf serum in RPMI-1640 medium .
	manualset3
145493	11	409352	5	NULL	NULL	0	NULL	RPMI-1640 medium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The culture medium included 10-100 units/ml of recombinant lymphokines ( rIL-1 , rIL-2 , rIL-4 , rIL-6 and rIL-7 ) and 10 % fetal calf serum in RPMI-1640 medium .
	manualset3
145494	1	409353	5	NULL	NULL	NULL	NULL	culture supernatant	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The culture supernatant of activated macrophages did not show any lytic activity .
	manualset3
145495	2	409353	5	NULL	NULL	0	NULL	activated macrophages 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The culture supernatant of activated macrophages did not show any lytic activity .
	manualset3
145496	3	409353	5	NULL	NULL	0	NULL	lytic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The culture supernatant of activated macrophages did not show any lytic activity .
	manualset3
145497	1	409354	5	NULL	NULL	0	NULL	cumulative incidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cumulative incidence of insulin-treated patients was 42 % at 8 years and reached 91 % at 14 years , but the progression to insulin dependence was very variable among the patients .
	manualset3
145498	2	409354	5	NULL	NULL	0	NULL	insulin-treated patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The cumulative incidence of insulin-treated patients was 42 % at 8 years and reached 91 % at 14 years , but the progression to insulin dependence was very variable among the patients .
	manualset3
145499	3	409354	5	NULL	NULL	0	NULL	42 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The cumulative incidence of insulin-treated patients was 42 % at 8 years and reached 91 % at 14 years , but the progression to insulin dependence was very variable among the patients .
	manualset3
145500	4	409354	5	NULL	NULL	0	NULL	8 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The cumulative incidence of insulin-treated patients was 42 % at 8 years and reached 91 % at 14 years , but the progression to insulin dependence was very variable among the patients .
	manualset3
145501	5	409354	5	NULL	NULL	0	NULL	91 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The cumulative incidence of insulin-treated patients was 42 % at 8 years and reached 91 % at 14 years , but the progression to insulin dependence was very variable among the patients .
	manualset3
145502	6	409354	5	NULL	NULL	0	NULL	14 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The cumulative incidence of insulin-treated patients was 42 % at 8 years and reached 91 % at 14 years , but the progression to insulin dependence was very variable among the patients .
	manualset3
145503	7	409354	5	NULL	NULL	0	NULL	progression 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cumulative incidence of insulin-treated patients was 42 % at 8 years and reached 91 % at 14 years , but the progression to insulin dependence was very variable among the patients .
	manualset3
145504	8	409354	5	NULL	NULL	NULL	NULL	insulin dependence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The cumulative incidence of insulin-treated patients was 42 % at 8 years and reached 91 % at 14 years , but the progression to insulin dependence was very variable among the patients .
	manualset3
145505	9	409354	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The cumulative incidence of insulin-treated patients was 42 % at 8 years and reached 91 % at 14 years , but the progression to insulin dependence was very variable among the patients .
	manualset3
145506	1	409355	5	NULL	NULL	0	NULL	levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The current allowable levels of EO on medical devices sterilized with EO gas as outlined in International Organization for Standardization ( ISO ) 10993-7 may be significantly reduced from current levels by applying the ISO Draft International Standard 10993-17 method for establishing allowable limits .
	manualset3
145507	2	409355	5	NULL	NULL	0	NULL	medical devices	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The current allowable levels of EO on medical devices sterilized with EO gas as outlined in International Organization for Standardization ( ISO ) 10993-7 may be significantly reduced from current levels by applying the ISO Draft International Standard 10993-17 method for establishing allowable limits .
	manualset3
145508	3	409355	5	NULL	NULL	0	NULL	EO gas	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The current allowable levels of EO on medical devices sterilized with EO gas as outlined in International Organization for Standardization ( ISO ) 10993-7 may be significantly reduced from current levels by applying the ISO Draft International Standard 10993-17 method for establishing allowable limits .
	manualset3
145509	4	409355	5	NULL	NULL	0	NULL	International Organization for Standardization ( ISO ) 10993-7 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The current allowable levels of EO on medical devices sterilized with EO gas as outlined in International Organization for Standardization ( ISO ) 10993-7 may be significantly reduced from current levels by applying the ISO Draft International Standard 10993-17 method for establishing allowable limits .
	manualset3
145510	5	409355	5	NULL	NULL	0	NULL	current levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The current allowable levels of EO on medical devices sterilized with EO gas as outlined in International Organization for Standardization ( ISO ) 10993-7 may be significantly reduced from current levels by applying the ISO Draft International Standard 10993-17 method for establishing allowable limits .
	manualset3
145511	6	409355	5	NULL	NULL	0	NULL	ISO Draft International Standard 10993-17 method 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The current allowable levels of EO on medical devices sterilized with EO gas as outlined in International Organization for Standardization ( ISO ) 10993-7 may be significantly reduced from current levels by applying the ISO Draft International Standard 10993-17 method for establishing allowable limits .
	manualset3
145512	7	409355	5	NULL	NULL	0	NULL	limits 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The current allowable levels of EO on medical devices sterilized with EO gas as outlined in International Organization for Standardization ( ISO ) 10993-7 may be significantly reduced from current levels by applying the ISO Draft International Standard 10993-17 method for establishing allowable limits .
	manualset3
145513	1	409356	5	NULL	NULL	0	NULL	current dose-response relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The current dose-response relationship between caries and extrinsic sugars suggests that the sugars levels above 60 g/person/day for teenagers and adults increases the rate of caries .
	manualset3
145514	2	409356	5	NULL	NULL	0	NULL	caries 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The current dose-response relationship between caries and extrinsic sugars suggests that the sugars levels above 60 g/person/day for teenagers and adults increases the rate of caries .
	manualset3
145515	3	409356	5	NULL	NULL	0	NULL	extrinsic sugars 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The current dose-response relationship between caries and extrinsic sugars suggests that the sugars levels above 60 g/person/day for teenagers and adults increases the rate of caries .
	manualset3
145516	4	409356	5	NULL	NULL	0	NULL	sugars levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The current dose-response relationship between caries and extrinsic sugars suggests that the sugars levels above 60 g/person/day for teenagers and adults increases the rate of caries .
	manualset3
145517	5	409356	5	NULL	NULL	0	NULL	60 g/person/day 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The current dose-response relationship between caries and extrinsic sugars suggests that the sugars levels above 60 g/person/day for teenagers and adults increases the rate of caries .
	manualset3
145518	6	409356	5	NULL	NULL	0	NULL	teenagers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The current dose-response relationship between caries and extrinsic sugars suggests that the sugars levels above 60 g/person/day for teenagers and adults increases the rate of caries .
	manualset3
145519	7	409356	5	NULL	NULL	0	NULL	adults 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The current dose-response relationship between caries and extrinsic sugars suggests that the sugars levels above 60 g/person/day for teenagers and adults increases the rate of caries .
	manualset3
145520	8	409356	5	NULL	NULL	0	NULL	rate 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The current dose-response relationship between caries and extrinsic sugars suggests that the sugars levels above 60 g/person/day for teenagers and adults increases the rate of caries .
	manualset3
145521	9	409356	5	NULL	NULL	0	NULL	caries 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The current dose-response relationship between caries and extrinsic sugars suggests that the sugars levels above 60 g/person/day for teenagers and adults increases the rate of caries .
	manualset3
145522	1	409357	5	NULL	NULL	0	NULL	reaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar reaction with ( ( n ) Bu ( 4 ) N ) ( HSCoM ) did not afford the corresponding trivalent HSCoM ( - ) adduct , but rather the divalent nickel complex polymer ( - Ni ( II ) ( cyclam ) ( CoMSSCoM ) - ) ( n ) was obtained , in which the terminal thiol of HSCoM ( - ) was oxidized to the disulfide ( CoMSSCoM ) ( 2 - ) by the Ni ( III ) center .
	manualset3
145523	2	409357	5	NULL	NULL	0	NULL	( ( n ) Bu ( 4 ) N ) ( HSCoM )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar reaction with ( ( n ) Bu ( 4 ) N ) ( HSCoM ) did not afford the corresponding trivalent HSCoM ( - ) adduct , but rather the divalent nickel complex polymer ( - Ni ( II ) ( cyclam ) ( CoMSSCoM ) - ) ( n ) was obtained , in which the terminal thiol of HSCoM ( - ) was oxidized to the disulfide ( CoMSSCoM ) ( 2 - ) by the Ni ( III ) center .
	manualset3
145524	3	409357	5	NULL	NULL	0	NULL	trivalent HSCoM ( - ) adduct	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar reaction with ( ( n ) Bu ( 4 ) N ) ( HSCoM ) did not afford the corresponding trivalent HSCoM ( - ) adduct , but rather the divalent nickel complex polymer ( - Ni ( II ) ( cyclam ) ( CoMSSCoM ) - ) ( n ) was obtained , in which the terminal thiol of HSCoM ( - ) was oxidized to the disulfide ( CoMSSCoM ) ( 2 - ) by the Ni ( III ) center .
	manualset3
145525	4	409357	5	NULL	NULL	0	NULL	divalent nickel complex polymer ( - Ni ( II ) ( cyclam ) ( CoMSSCoM ) - ) ( n )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar reaction with ( ( n ) Bu ( 4 ) N ) ( HSCoM ) did not afford the corresponding trivalent HSCoM ( - ) adduct , but rather the divalent nickel complex polymer ( - Ni ( II ) ( cyclam ) ( CoMSSCoM ) - ) ( n ) was obtained , in which the terminal thiol of HSCoM ( - ) was oxidized to the disulfide ( CoMSSCoM ) ( 2 - ) by the Ni ( III ) center .
	manualset3
145526	5	409357	5	NULL	NULL	0	NULL	terminal thiol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar reaction with ( ( n ) Bu ( 4 ) N ) ( HSCoM ) did not afford the corresponding trivalent HSCoM ( - ) adduct , but rather the divalent nickel complex polymer ( - Ni ( II ) ( cyclam ) ( CoMSSCoM ) - ) ( n ) was obtained , in which the terminal thiol of HSCoM ( - ) was oxidized to the disulfide ( CoMSSCoM ) ( 2 - ) by the Ni ( III ) center .
	manualset3
145527	6	409357	5	NULL	NULL	0	NULL	HSCoM ( - ) 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar reaction with ( ( n ) Bu ( 4 ) N ) ( HSCoM ) did not afford the corresponding trivalent HSCoM ( - ) adduct , but rather the divalent nickel complex polymer ( - Ni ( II ) ( cyclam ) ( CoMSSCoM ) - ) ( n ) was obtained , in which the terminal thiol of HSCoM ( - ) was oxidized to the disulfide ( CoMSSCoM ) ( 2 - ) by the Ni ( III ) center .
	manualset3
145528	7	409357	5	NULL	NULL	0	NULL	disulfide ( CoMSSCoM ) ( 2 - )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar reaction with ( ( n ) Bu ( 4 ) N ) ( HSCoM ) did not afford the corresponding trivalent HSCoM ( - ) adduct , but rather the divalent nickel complex polymer ( - Ni ( II ) ( cyclam ) ( CoMSSCoM ) - ) ( n ) was obtained , in which the terminal thiol of HSCoM ( - ) was oxidized to the disulfide ( CoMSSCoM ) ( 2 - ) by the Ni ( III ) center .
	manualset3
145529	8	409357	5	NULL	NULL	0	NULL	Ni ( III ) center	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar reaction with ( ( n ) Bu ( 4 ) N ) ( HSCoM ) did not afford the corresponding trivalent HSCoM ( - ) adduct , but rather the divalent nickel complex polymer ( - Ni ( II ) ( cyclam ) ( CoMSSCoM ) - ) ( n ) was obtained , in which the terminal thiol of HSCoM ( - ) was oxidized to the disulfide ( CoMSSCoM ) ( 2 - ) by the Ni ( III ) center .
	manualset3
145530	1	409358	5	NULL	NULL	0	NULL	current findings	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The current findings add to a nascent empirical literature suggesting that aberrant processing of positive social information may contribute to the persistence of excessive social anxiety .
	manualset3
145531	2	409358	5	NULL	NULL	0	NULL	nascent empirical literature 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The current findings add to a nascent empirical literature suggesting that aberrant processing of positive social information may contribute to the persistence of excessive social anxiety .
	manualset3
145532	3	409358	5	NULL	NULL	0	NULL	aberrant processing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The current findings add to a nascent empirical literature suggesting that aberrant processing of positive social information may contribute to the persistence of excessive social anxiety .
	manualset3
145533	4	409358	5	NULL	NULL	0	NULL	positive social information	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The current findings add to a nascent empirical literature suggesting that aberrant processing of positive social information may contribute to the persistence of excessive social anxiety .
	manualset3
145534	5	409358	5	NULL	NULL	0	NULL	excessive social anxiety	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The current findings add to a nascent empirical literature suggesting that aberrant processing of positive social information may contribute to the persistence of excessive social anxiety .
	manualset3
145535	1	409359	5	NULL	NULL	0	NULL	current guidelines	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The current guidelines were deliberated beforehand by a number of physicians that are recognized for their expertise on the subject , coming from the specialities of endocrinology ( the French Thyroid Research Group ) and surgery ( the French Association for Endocrine Surgery ) , as well as representatives from the fields of biology , ultrasonography , cytology and nuclear medicine .
	manualset3
145536	2	409359	5	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The current guidelines were deliberated beforehand by a number of physicians that are recognized for their expertise on the subject , coming from the specialities of endocrinology ( the French Thyroid Research Group ) and surgery ( the French Association for Endocrine Surgery ) , as well as representatives from the fields of biology , ultrasonography , cytology and nuclear medicine .
	manualset3
145537	3	409359	5	NULL	NULL	0	NULL	physicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The current guidelines were deliberated beforehand by a number of physicians that are recognized for their expertise on the subject , coming from the specialities of endocrinology ( the French Thyroid Research Group ) and surgery ( the French Association for Endocrine Surgery ) , as well as representatives from the fields of biology , ultrasonography , cytology and nuclear medicine .
	manualset3
145538	4	409359	5	NULL	NULL	0	NULL	expertise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The current guidelines were deliberated beforehand by a number of physicians that are recognized for their expertise on the subject , coming from the specialities of endocrinology ( the French Thyroid Research Group ) and surgery ( the French Association for Endocrine Surgery ) , as well as representatives from the fields of biology , ultrasonography , cytology and nuclear medicine .
	manualset3
145539	5	409359	5	NULL	NULL	0	NULL	subject	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The current guidelines were deliberated beforehand by a number of physicians that are recognized for their expertise on the subject , coming from the specialities of endocrinology ( the French Thyroid Research Group ) and surgery ( the French Association for Endocrine Surgery ) , as well as representatives from the fields of biology , ultrasonography , cytology and nuclear medicine .
	manualset3
145540	6	409359	5	NULL	NULL	0	NULL	specialities	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The current guidelines were deliberated beforehand by a number of physicians that are recognized for their expertise on the subject , coming from the specialities of endocrinology ( the French Thyroid Research Group ) and surgery ( the French Association for Endocrine Surgery ) , as well as representatives from the fields of biology , ultrasonography , cytology and nuclear medicine .
	manualset3
145541	7	409359	5	NULL	NULL	0	NULL	endocrinology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The current guidelines were deliberated beforehand by a number of physicians that are recognized for their expertise on the subject , coming from the specialities of endocrinology ( the French Thyroid Research Group ) and surgery ( the French Association for Endocrine Surgery ) , as well as representatives from the fields of biology , ultrasonography , cytology and nuclear medicine .
	manualset3
145542	8	409359	5	NULL	NULL	0	NULL	French Thyroid Research Group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The current guidelines were deliberated beforehand by a number of physicians that are recognized for their expertise on the subject , coming from the specialities of endocrinology ( the French Thyroid Research Group ) and surgery ( the French Association for Endocrine Surgery ) , as well as representatives from the fields of biology , ultrasonography , cytology and nuclear medicine .
	manualset3
145543	9	409359	5	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The current guidelines were deliberated beforehand by a number of physicians that are recognized for their expertise on the subject , coming from the specialities of endocrinology ( the French Thyroid Research Group ) and surgery ( the French Association for Endocrine Surgery ) , as well as representatives from the fields of biology , ultrasonography , cytology and nuclear medicine .
	manualset3
145544	10	409359	5	NULL	NULL	0	NULL	French Association for Endocrine Surgery	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The current guidelines were deliberated beforehand by a number of physicians that are recognized for their expertise on the subject , coming from the specialities of endocrinology ( the French Thyroid Research Group ) and surgery ( the French Association for Endocrine Surgery ) , as well as representatives from the fields of biology , ultrasonography , cytology and nuclear medicine .
	manualset3
145545	11	409359	5	NULL	NULL	0	NULL	representatives	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The current guidelines were deliberated beforehand by a number of physicians that are recognized for their expertise on the subject , coming from the specialities of endocrinology ( the French Thyroid Research Group ) and surgery ( the French Association for Endocrine Surgery ) , as well as representatives from the fields of biology , ultrasonography , cytology and nuclear medicine .
	manualset3
145546	12	409359	5	NULL	NULL	0	NULL	fields of biology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The current guidelines were deliberated beforehand by a number of physicians that are recognized for their expertise on the subject , coming from the specialities of endocrinology ( the French Thyroid Research Group ) and surgery ( the French Association for Endocrine Surgery ) , as well as representatives from the fields of biology , ultrasonography , cytology and nuclear medicine .
	manualset3
145547	13	409359	5	NULL	NULL	0	NULL	ultrasonography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The current guidelines were deliberated beforehand by a number of physicians that are recognized for their expertise on the subject , coming from the specialities of endocrinology ( the French Thyroid Research Group ) and surgery ( the French Association for Endocrine Surgery ) , as well as representatives from the fields of biology , ultrasonography , cytology and nuclear medicine .
	manualset3
145548	14	409359	5	NULL	NULL	0	NULL	cytology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The current guidelines were deliberated beforehand by a number of physicians that are recognized for their expertise on the subject , coming from the specialities of endocrinology ( the French Thyroid Research Group ) and surgery ( the French Association for Endocrine Surgery ) , as well as representatives from the fields of biology , ultrasonography , cytology and nuclear medicine .
	manualset3
145549	15	409359	5	NULL	NULL	0	NULL	nuclear medicine	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The current guidelines were deliberated beforehand by a number of physicians that are recognized for their expertise on the subject , coming from the specialities of endocrinology ( the French Thyroid Research Group ) and surgery ( the French Association for Endocrine Surgery ) , as well as representatives from the fields of biology , ultrasonography , cytology and nuclear medicine .
	manualset3
145550	1	409360	5	NULL	NULL	0	NULL	current model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The current model suggests that superoxide generated by CeDUOX1 at the C-terminal NADPH oxidase domain is rapidly converted to H ( 2 ) O ( 2 ) .
	manualset3
145551	2	409360	5	NULL	NULL	0	NULL	superoxide	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The current model suggests that superoxide generated by CeDUOX1 at the C-terminal NADPH oxidase domain is rapidly converted to H ( 2 ) O ( 2 ) .
	manualset3
145552	3	409360	5	NULL	NULL	0	NULL	CeDUOX1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The current model suggests that superoxide generated by CeDUOX1 at the C-terminal NADPH oxidase domain is rapidly converted to H ( 2 ) O ( 2 ) .
	manualset3
145553	4	409360	5	NULL	NULL	0	NULL	C-terminal NADPH oxidase domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The current model suggests that superoxide generated by CeDUOX1 at the C-terminal NADPH oxidase domain is rapidly converted to H ( 2 ) O ( 2 ) .
	manualset3
145554	5	409360	5	NULL	NULL	0	NULL	H ( 2 ) O ( 2 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The current model suggests that superoxide generated by CeDUOX1 at the C-terminal NADPH oxidase domain is rapidly converted to H ( 2 ) O ( 2 ) .
	manualset3
145555	1	409361	5	NULL	NULL	0	NULL	current nomenclature	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The current nomenclature , potential therapeutic effects and importance of 5-HT receptor subtype antagonism will be examined .
	manualset3
145556	2	409361	5	NULL	NULL	0	NULL	potential therapeutic effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The current nomenclature , potential therapeutic effects and importance of 5-HT receptor subtype antagonism will be examined .
	manualset3
145557	3	409361	5	NULL	NULL	0	NULL	importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The current nomenclature , potential therapeutic effects and importance of 5-HT receptor subtype antagonism will be examined .
	manualset3
145558	4	409361	5	NULL	NULL	0	NULL	5-HT receptor subtype antagonism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The current nomenclature , potential therapeutic effects and importance of 5-HT receptor subtype antagonism will be examined .
	manualset3
145559	1	409362	5	NULL	NULL	0	NULL	current paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The current paper reports an 8 year old girl with arthralgia and polyclonal B cell activation induced by human parvovirus B19 infection ( HPV B19 ) .
	manualset3
145560	2	409362	5	NULL	NULL	0	NULL	8 year old girl 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The current paper reports an 8 year old girl with arthralgia and polyclonal B cell activation induced by human parvovirus B19 infection ( HPV B19 ) .
	manualset3
145561	3	409362	5	NULL	NULL	0	NULL	arthralgia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The current paper reports an 8 year old girl with arthralgia and polyclonal B cell activation induced by human parvovirus B19 infection ( HPV B19 ) .
	manualset3
145562	4	409362	5	NULL	NULL	0	NULL	polyclonal B cell activation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The current paper reports an 8 year old girl with arthralgia and polyclonal B cell activation induced by human parvovirus B19 infection ( HPV B19 ) .
	manualset3
145563	5	409362	5	NULL	NULL	0	NULL	human parvovirus B19 infection ( HPV B19 )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The current paper reports an 8 year old girl with arthralgia and polyclonal B cell activation induced by human parvovirus B19 infection ( HPV B19 ) .
	manualset3
145564	1	409363	5	NULL	NULL	0	NULL	practice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The current practice of German psychiatric hospitals restricts electroconvulsive therapy ( ECT ) to patients with profound disability and failure to respond to pharmacotherapy .
	manualset3
145565	2	409363	5	NULL	NULL	0	NULL	German psychiatric hospitals	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The current practice of German psychiatric hospitals restricts electroconvulsive therapy ( ECT ) to patients with profound disability and failure to respond to pharmacotherapy .
	manualset3
145566	3	409363	5	NULL	NULL	0	NULL	electroconvulsive therapy ( ECT )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The current practice of German psychiatric hospitals restricts electroconvulsive therapy ( ECT ) to patients with profound disability and failure to respond to pharmacotherapy .
	manualset3
145567	4	409363	5	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The current practice of German psychiatric hospitals restricts electroconvulsive therapy ( ECT ) to patients with profound disability and failure to respond to pharmacotherapy .
	manualset3
145568	5	409363	5	NULL	NULL	0	NULL	disability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The current practice of German psychiatric hospitals restricts electroconvulsive therapy ( ECT ) to patients with profound disability and failure to respond to pharmacotherapy .
	manualset3
145569	6	409363	5	NULL	NULL	NULL	NULL	failure	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The current practice of German psychiatric hospitals restricts electroconvulsive therapy ( ECT ) to patients with profound disability and failure to respond to pharmacotherapy .
	manualset3
145570	7	409363	5	NULL	NULL	0	NULL	pharmacotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The current practice of German psychiatric hospitals restricts electroconvulsive therapy ( ECT ) to patients with profound disability and failure to respond to pharmacotherapy .
	manualset3
145571	1	409364	5	NULL	NULL	0	NULL	current problem	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The current problem of acupuncture and moxibustion education is that incomplete and unsystematic content , simple and boring teaching method , and poor-level training in clinical practice .
	manualset3
145572	2	409364	5	NULL	NULL	0	NULL	acupuncture	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The current problem of acupuncture and moxibustion education is that incomplete and unsystematic content , simple and boring teaching method , and poor-level training in clinical practice .
	manualset3
145573	3	409364	5	NULL	NULL	0	NULL	moxibustion education	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The current problem of acupuncture and moxibustion education is that incomplete and unsystematic content , simple and boring teaching method , and poor-level training in clinical practice .
	manualset3
145574	4	409364	5	NULL	NULL	0	NULL	content	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The current problem of acupuncture and moxibustion education is that incomplete and unsystematic content , simple and boring teaching method , and poor-level training in clinical practice .
	manualset3
145575	5	409364	5	NULL	NULL	0	NULL	teaching method	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The current problem of acupuncture and moxibustion education is that incomplete and unsystematic content , simple and boring teaching method , and poor-level training in clinical practice .
	manualset3
145576	6	409364	5	NULL	NULL	0	NULL	training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The current problem of acupuncture and moxibustion education is that incomplete and unsystematic content , simple and boring teaching method , and poor-level training in clinical practice .
	manualset3
145577	7	409364	5	NULL	NULL	0	NULL	clinical practice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The current problem of acupuncture and moxibustion education is that incomplete and unsystematic content , simple and boring teaching method , and poor-level training in clinical practice .
	manualset3
145578	1	409365	5	NULL	NULL	0	NULL	current special issue	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The current special issue focuses on topics relevant for integrating this research within the broader literature on childhood psychopathology .
	manualset3
145579	2	409365	5	NULL	NULL	0	NULL	topics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The current special issue focuses on topics relevant for integrating this research within the broader literature on childhood psychopathology .
	manualset3
145580	3	409365	5	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The current special issue focuses on topics relevant for integrating this research within the broader literature on childhood psychopathology .
	manualset3
145581	4	409365	5	NULL	NULL	0	NULL	literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The current special issue focuses on topics relevant for integrating this research within the broader literature on childhood psychopathology .
	manualset3
145582	5	409365	5	NULL	NULL	0	NULL	childhood psychopathology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The current special issue focuses on topics relevant for integrating this research within the broader literature on childhood psychopathology .
	manualset3
145583	1	409366	5	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The current studies examine acetaminophen pharmacokinetics and biotransformation in obese animals for possible shifts in metabolic conjugation reactions .
	manualset3
145584	2	409366	5	NULL	NULL	0	NULL	acetaminophen	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The current studies examine acetaminophen pharmacokinetics and biotransformation in obese animals for possible shifts in metabolic conjugation reactions .
	manualset3
145585	3	409366	5	NULL	NULL	0	NULL	pharmacokinetics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The current studies examine acetaminophen pharmacokinetics and biotransformation in obese animals for possible shifts in metabolic conjugation reactions .
	manualset3
145586	4	409366	5	NULL	NULL	0	NULL	biotransformation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The current studies examine acetaminophen pharmacokinetics and biotransformation in obese animals for possible shifts in metabolic conjugation reactions .
	manualset3
145587	5	409366	5	NULL	NULL	0	NULL	obese animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The current studies examine acetaminophen pharmacokinetics and biotransformation in obese animals for possible shifts in metabolic conjugation reactions .
	manualset3
145588	6	409366	5	NULL	NULL	0	NULL	shifts	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The current studies examine acetaminophen pharmacokinetics and biotransformation in obese animals for possible shifts in metabolic conjugation reactions .
	manualset3
145589	7	409366	5	NULL	NULL	0	NULL	metabolic conjugation reactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The current studies examine acetaminophen pharmacokinetics and biotransformation in obese animals for possible shifts in metabolic conjugation reactions .
	manualset3
145590	1	409367	5	NULL	NULL	0	NULL	series of peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar series of peptides based upon human rhinovirus 3C cleavage sites was also examined .
	manualset3
145591	2	409367	5	NULL	NULL	0	NULL	human rhinovirus 3C cleavage sites 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar series of peptides based upon human rhinovirus 3C cleavage sites was also examined .
	manualset3
145592	1	409368	5	NULL	NULL	0	NULL	current study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study analyzed the relationship between text comprehension and memory skills in preschoolers .
	manualset3
145593	2	409368	5	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study analyzed the relationship between text comprehension and memory skills in preschoolers .
	manualset3
145594	3	409368	5	NULL	NULL	0	NULL	text comprehension	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study analyzed the relationship between text comprehension and memory skills in preschoolers .
	manualset3
145595	4	409368	5	NULL	NULL	0	NULL	memory skills	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study analyzed the relationship between text comprehension and memory skills in preschoolers .
	manualset3
145596	5	409368	5	NULL	NULL	0	NULL	preschoolers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study analyzed the relationship between text comprehension and memory skills in preschoolers .
	manualset3
145597	1	409369	5	NULL	NULL	0	NULL	current study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study examined the association between avoidance of conflict and measures of loneliness , social anxiety , and social avoidance for 59 pupils in Grade 4 ( 31 boys and 28 girls ) and 47 in Grade 8 ( 22 boys and 25 girls ) .
	manualset3
145598	2	409369	5	NULL	NULL	NULL	NULL	association	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The current study examined the association between avoidance of conflict and measures of loneliness , social anxiety , and social avoidance for 59 pupils in Grade 4 ( 31 boys and 28 girls ) and 47 in Grade 8 ( 22 boys and 25 girls ) .
	manualset3
145599	3	409369	5	NULL	NULL	0	NULL	avoidance of conflict	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study examined the association between avoidance of conflict and measures of loneliness , social anxiety , and social avoidance for 59 pupils in Grade 4 ( 31 boys and 28 girls ) and 47 in Grade 8 ( 22 boys and 25 girls ) .
	manualset3
145600	4	409369	5	NULL	NULL	0	NULL	measures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study examined the association between avoidance of conflict and measures of loneliness , social anxiety , and social avoidance for 59 pupils in Grade 4 ( 31 boys and 28 girls ) and 47 in Grade 8 ( 22 boys and 25 girls ) .
	manualset3
145601	5	409369	5	NULL	NULL	0	NULL	loneliness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study examined the association between avoidance of conflict and measures of loneliness , social anxiety , and social avoidance for 59 pupils in Grade 4 ( 31 boys and 28 girls ) and 47 in Grade 8 ( 22 boys and 25 girls ) .
	manualset3
145602	6	409369	5	NULL	NULL	0	NULL	social anxiety	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study examined the association between avoidance of conflict and measures of loneliness , social anxiety , and social avoidance for 59 pupils in Grade 4 ( 31 boys and 28 girls ) and 47 in Grade 8 ( 22 boys and 25 girls ) .
	manualset3
145603	7	409369	5	NULL	NULL	0	NULL	social avoidance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study examined the association between avoidance of conflict and measures of loneliness , social anxiety , and social avoidance for 59 pupils in Grade 4 ( 31 boys and 28 girls ) and 47 in Grade 8 ( 22 boys and 25 girls ) .
	manualset3
145604	8	409369	5	NULL	NULL	0	NULL	59 pupils	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study examined the association between avoidance of conflict and measures of loneliness , social anxiety , and social avoidance for 59 pupils in Grade 4 ( 31 boys and 28 girls ) and 47 in Grade 8 ( 22 boys and 25 girls ) .
	manualset3
145605	9	409369	5	NULL	NULL	0	NULL	Grade 4	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study examined the association between avoidance of conflict and measures of loneliness , social anxiety , and social avoidance for 59 pupils in Grade 4 ( 31 boys and 28 girls ) and 47 in Grade 8 ( 22 boys and 25 girls ) .
	manualset3
145606	10	409369	5	NULL	NULL	0	NULL	31 boys	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study examined the association between avoidance of conflict and measures of loneliness , social anxiety , and social avoidance for 59 pupils in Grade 4 ( 31 boys and 28 girls ) and 47 in Grade 8 ( 22 boys and 25 girls ) .
	manualset3
145607	11	409369	5	NULL	NULL	0	NULL	28 girls	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study examined the association between avoidance of conflict and measures of loneliness , social anxiety , and social avoidance for 59 pupils in Grade 4 ( 31 boys and 28 girls ) and 47 in Grade 8 ( 22 boys and 25 girls ) .
	manualset3
145608	12	409369	5	NULL	NULL	0	NULL	47	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study examined the association between avoidance of conflict and measures of loneliness , social anxiety , and social avoidance for 59 pupils in Grade 4 ( 31 boys and 28 girls ) and 47 in Grade 8 ( 22 boys and 25 girls ) .
	manualset3
145609	13	409369	5	NULL	NULL	0	NULL	Grade 8	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study examined the association between avoidance of conflict and measures of loneliness , social anxiety , and social avoidance for 59 pupils in Grade 4 ( 31 boys and 28 girls ) and 47 in Grade 8 ( 22 boys and 25 girls ) .
	manualset3
145610	14	409369	5	NULL	NULL	0	NULL	22 boys	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study examined the association between avoidance of conflict and measures of loneliness , social anxiety , and social avoidance for 59 pupils in Grade 4 ( 31 boys and 28 girls ) and 47 in Grade 8 ( 22 boys and 25 girls ) .
	manualset3
145611	15	409369	5	NULL	NULL	0	NULL	25 girls	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study examined the association between avoidance of conflict and measures of loneliness , social anxiety , and social avoidance for 59 pupils in Grade 4 ( 31 boys and 28 girls ) and 47 in Grade 8 ( 22 boys and 25 girls ) .
	manualset3
145612	1	409370	5	NULL	NULL	0	NULL	current study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study focused on two aspects of health maintenance for families : advocacy and practice .
	manualset3
145613	2	409370	5	NULL	NULL	0	NULL	 two aspects	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study focused on two aspects of health maintenance for families : advocacy and practice .
	manualset3
145614	3	409370	5	NULL	NULL	0	NULL	health maintenance	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study focused on two aspects of health maintenance for families : advocacy and practice .
	manualset3
145615	4	409370	5	NULL	NULL	0	NULL	families	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study focused on two aspects of health maintenance for families : advocacy and practice .
	manualset3
145616	5	409370	5	NULL	NULL	0	NULL	advocacy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study focused on two aspects of health maintenance for families : advocacy and practice .
	manualset3
145617	6	409370	5	NULL	NULL	0	NULL	practice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study focused on two aspects of health maintenance for families : advocacy and practice .
	manualset3
145618	1	409371	5	NULL	NULL	0	NULL	current study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study investigated whether exposure with response prevention ( ERP ) for obsessive compulsive disorder ( OCD ) is more effective when administered in a participant 's home or other natural environments where symptoms tend to occur , than in a therapist 's office .
	manualset3
145619	2	409371	5	NULL	NULL	NULL	NULL	exposure with response prevention ( ERP )	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The current study investigated whether exposure with response prevention ( ERP ) for obsessive compulsive disorder ( OCD ) is more effective when administered in a participant 's home or other natural environments where symptoms tend to occur , than in a therapist 's office .
	manualset3
145620	3	409371	5	NULL	NULL	0	NULL	obsessive compulsive disorder ( OCD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study investigated whether exposure with response prevention ( ERP ) for obsessive compulsive disorder ( OCD ) is more effective when administered in a participant 's home or other natural environments where symptoms tend to occur , than in a therapist 's office .
	manualset3
145622	5	409371	5	NULL	NULL	0	NULL	participant	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study investigated whether exposure with response prevention ( ERP ) for obsessive compulsive disorder ( OCD ) is more effective when administered in a participant 's home or other natural environments where symptoms tend to occur , than in a therapist 's office .
	manualset3
145623	6	409371	5	NULL	NULL	0	NULL	home	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study investigated whether exposure with response prevention ( ERP ) for obsessive compulsive disorder ( OCD ) is more effective when administered in a participant 's home or other natural environments where symptoms tend to occur , than in a therapist 's office .
	manualset3
145624	7	409371	5	NULL	NULL	0	NULL	natural environments	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study investigated whether exposure with response prevention ( ERP ) for obsessive compulsive disorder ( OCD ) is more effective when administered in a participant 's home or other natural environments where symptoms tend to occur , than in a therapist 's office .
	manualset3
145625	8	409371	5	NULL	NULL	0	NULL	symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study investigated whether exposure with response prevention ( ERP ) for obsessive compulsive disorder ( OCD ) is more effective when administered in a participant 's home or other natural environments where symptoms tend to occur , than in a therapist 's office .
	manualset3
145626	9	409371	5	NULL	NULL	0	NULL	therapist	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study investigated whether exposure with response prevention ( ERP ) for obsessive compulsive disorder ( OCD ) is more effective when administered in a participant 's home or other natural environments where symptoms tend to occur , than in a therapist 's office .
	manualset3
145627	10	409371	5	NULL	NULL	0	NULL	office	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study investigated whether exposure with response prevention ( ERP ) for obsessive compulsive disorder ( OCD ) is more effective when administered in a participant 's home or other natural environments where symptoms tend to occur , than in a therapist 's office .
	manualset3
145628	1	409372	5	NULL	NULL	0	NULL	current study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study suggested that the binding capacities of DesIgA1 and Des/DeGalIgA1 to HMC were significantly higher than that of normal IgA1 , which at least in part was due to more macromolecular IgA1 in deglycoslated IgA1 .
	manualset3
145629	2	409372	5	NULL	NULL	0	NULL	binding capacities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study suggested that the binding capacities of DesIgA1 and Des/DeGalIgA1 to HMC were significantly higher than that of normal IgA1 , which at least in part was due to more macromolecular IgA1 in deglycoslated IgA1 .
	manualset3
145630	3	409372	5	NULL	NULL	0	NULL	DesIgA1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study suggested that the binding capacities of DesIgA1 and Des/DeGalIgA1 to HMC were significantly higher than that of normal IgA1 , which at least in part was due to more macromolecular IgA1 in deglycoslated IgA1 .
	manualset3
145631	4	409372	5	NULL	NULL	0	NULL	Des/DeGalIgA1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study suggested that the binding capacities of DesIgA1 and Des/DeGalIgA1 to HMC were significantly higher than that of normal IgA1 , which at least in part was due to more macromolecular IgA1 in deglycoslated IgA1 .
	manualset3
145632	5	409372	5	NULL	NULL	0	NULL	HMC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study suggested that the binding capacities of DesIgA1 and Des/DeGalIgA1 to HMC were significantly higher than that of normal IgA1 , which at least in part was due to more macromolecular IgA1 in deglycoslated IgA1 .
	manualset3
145633	6	409372	5	NULL	NULL	0	NULL	normal IgA1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study suggested that the binding capacities of DesIgA1 and Des/DeGalIgA1 to HMC were significantly higher than that of normal IgA1 , which at least in part was due to more macromolecular IgA1 in deglycoslated IgA1 .
	manualset3
145634	7	409372	5	NULL	NULL	0	NULL	macromolecular IgA1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study suggested that the binding capacities of DesIgA1 and Des/DeGalIgA1 to HMC were significantly higher than that of normal IgA1 , which at least in part was due to more macromolecular IgA1 in deglycoslated IgA1 .
	manualset3
145635	8	409372	5	NULL	NULL	0	NULL	deglycoslated IgA1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The current study suggested that the binding capacities of DesIgA1 and Des/DeGalIgA1 to HMC were significantly higher than that of normal IgA1 , which at least in part was due to more macromolecular IgA1 in deglycoslated IgA1 .
	manualset3
145636	1	409373	5	NULL	NULL	0	NULL	validity study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The current validity study required five experienced clinicians to rank a total of 50 cases as having Low , Medium , or High Support Need based on descriptions that were part of an assessment package for services .
	manualset3
145637	2	409373	5	NULL	NULL	0	NULL	five	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The current validity study required five experienced clinicians to rank a total of 50 cases as having Low , Medium , or High Support Need based on descriptions that were part of an assessment package for services .
	manualset3
145638	3	409373	5	NULL	NULL	0	NULL	experienced clinicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The current validity study required five experienced clinicians to rank a total of 50 cases as having Low , Medium , or High Support Need based on descriptions that were part of an assessment package for services .
	manualset3
145639	4	409373	5	NULL	NULL	0	NULL	total	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The current validity study required five experienced clinicians to rank a total of 50 cases as having Low , Medium , or High Support Need based on descriptions that were part of an assessment package for services .
	manualset3
145640	5	409373	5	NULL	NULL	0	NULL	50 cases	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The current validity study required five experienced clinicians to rank a total of 50 cases as having Low , Medium , or High Support Need based on descriptions that were part of an assessment package for services .
	manualset3
145641	6	409373	5	NULL	NULL	0	NULL	Support Need	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The current validity study required five experienced clinicians to rank a total of 50 cases as having Low , Medium , or High Support Need based on descriptions that were part of an assessment package for services .
	manualset3
145642	7	409373	5	NULL	NULL	0	NULL	descriptions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The current validity study required five experienced clinicians to rank a total of 50 cases as having Low , Medium , or High Support Need based on descriptions that were part of an assessment package for services .
	manualset3
145643	8	409373	5	NULL	NULL	0	NULL	assessment package	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The current validity study required five experienced clinicians to rank a total of 50 cases as having Low , Medium , or High Support Need based on descriptions that were part of an assessment package for services .
	manualset3
145644	9	409373	5	NULL	NULL	0	NULL	services	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The current validity study required five experienced clinicians to rank a total of 50 cases as having Low , Medium , or High Support Need based on descriptions that were part of an assessment package for services .
	manualset3
145645	1	409374	5	NULL	NULL	0	NULL	countermeasures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The currently available and theoretically possible countermeasures against DCS in cosmonauts during EVA are considered .
	manualset3
145646	2	409374	5	NULL	NULL	0	NULL	DCS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The currently available and theoretically possible countermeasures against DCS in cosmonauts during EVA are considered .
	manualset3
145647	3	409374	5	NULL	NULL	0	NULL	cosmonauts	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The currently available and theoretically possible countermeasures against DCS in cosmonauts during EVA are considered .
	manualset3
145648	4	409374	5	NULL	NULL	0	NULL	EVA	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The currently available and theoretically possible countermeasures against DCS in cosmonauts during EVA are considered .
	manualset3
145649	1	409375	5	NULL	NULL	0	NULL	mutation analysis panel	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The currently available mutation analysis panel detects about 50-60 % of CFTR mutations in Hispanic patients .
	manualset3
145650	2	409375	5	NULL	NULL	0	NULL	50-60 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The currently available mutation analysis panel detects about 50-60 % of CFTR mutations in Hispanic patients .
	manualset3
145651	3	409375	5	NULL	NULL	0	NULL	CFTR mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The currently available mutation analysis panel detects about 50-60 % of CFTR mutations in Hispanic patients .
	manualset3
145652	4	409375	5	NULL	NULL	0	NULL	Hispanic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The currently available mutation analysis panel detects about 50-60 % of CFTR mutations in Hispanic patients .
	manualset3
145653	1	409376	5	NULL	NULL	0	NULL	curriculum	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The curriculum outlined by the WHO Curriculum Planning Group detailed the broad thrust of the Family Health Nurse Education Programme and was modified to be responsive to the context in which it was delivered , while staying faithful to general principles and precepts .
	manualset3
145654	2	409376	5	NULL	NULL	0	NULL	WHO Curriculum Planning Group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The curriculum outlined by the WHO Curriculum Planning Group detailed the broad thrust of the Family Health Nurse Education Programme and was modified to be responsive to the context in which it was delivered , while staying faithful to general principles and precepts .
	manualset3
145655	3	409376	5	NULL	NULL	0	NULL	broad thrust	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The curriculum outlined by the WHO Curriculum Planning Group detailed the broad thrust of the Family Health Nurse Education Programme and was modified to be responsive to the context in which it was delivered , while staying faithful to general principles and precepts .
	manualset3
145656	4	409376	5	NULL	NULL	0	NULL	Family Health Nurse Education Programme	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The curriculum outlined by the WHO Curriculum Planning Group detailed the broad thrust of the Family Health Nurse Education Programme and was modified to be responsive to the context in which it was delivered , while staying faithful to general principles and precepts .
	manualset3
145657	5	409376	5	NULL	NULL	0	NULL	responsive	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The curriculum outlined by the WHO Curriculum Planning Group detailed the broad thrust of the Family Health Nurse Education Programme and was modified to be responsive to the context in which it was delivered , while staying faithful to general principles and precepts .
	manualset3
145658	6	409376	5	NULL	NULL	0	NULL	context	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The curriculum outlined by the WHO Curriculum Planning Group detailed the broad thrust of the Family Health Nurse Education Programme and was modified to be responsive to the context in which it was delivered , while staying faithful to general principles and precepts .
	manualset3
145659	7	409376	5	NULL	NULL	0	NULL	general principles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The curriculum outlined by the WHO Curriculum Planning Group detailed the broad thrust of the Family Health Nurse Education Programme and was modified to be responsive to the context in which it was delivered , while staying faithful to general principles and precepts .
	manualset3
145660	8	409376	5	NULL	NULL	0	NULL	precepts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The curriculum outlined by the WHO Curriculum Planning Group detailed the broad thrust of the Family Health Nurse Education Programme and was modified to be responsive to the context in which it was delivered , while staying faithful to general principles and precepts .
	manualset3
145661	1	409377	5	NULL	NULL	0	NULL	soot ( TOR ) record	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar soot ( TOR ) record was also obtained from Lake Taihu ( ~ 200 km away ) , suggesting a regional source of soot .
	manualset3
145662	2	409377	5	NULL	NULL	0	NULL	Lake Taihu	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar soot ( TOR ) record was also obtained from Lake Taihu ( ~ 200 km away ) , suggesting a regional source of soot .
	manualset3
145663	3	409377	5	NULL	NULL	0	NULL	~ 200 km	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar soot ( TOR ) record was also obtained from Lake Taihu ( ~ 200 km away ) , suggesting a regional source of soot .
	manualset3
145664	4	409377	5	NULL	NULL	0	NULL	regional source	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar soot ( TOR ) record was also obtained from Lake Taihu ( ~ 200 km away ) , suggesting a regional source of soot .
	manualset3
145665	5	409377	5	NULL	NULL	0	NULL	soot	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A similar soot ( TOR ) record was also obtained from Lake Taihu ( ~ 200 km away ) , suggesting a regional source of soot .
	manualset3
145666	1	409378	5	NULL	NULL	0	NULL	telephone call	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The customary telephone call between resident and attending physician benefited from the additional photographic data , and patient management resulted in a clear , concise , and unambiguous treatment plan .
	manualset3
145667	2	409378	5	NULL	NULL	0	NULL	resident	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The customary telephone call between resident and attending physician benefited from the additional photographic data , and patient management resulted in a clear , concise , and unambiguous treatment plan .
	manualset3
145668	3	409378	5	NULL	NULL	0	NULL	attending physician	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The customary telephone call between resident and attending physician benefited from the additional photographic data , and patient management resulted in a clear , concise , and unambiguous treatment plan .
	manualset3
145669	4	409378	5	NULL	NULL	0	NULL	additional photographic data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The customary telephone call between resident and attending physician benefited from the additional photographic data , and patient management resulted in a clear , concise , and unambiguous treatment plan .
	manualset3
145670	5	409378	5	NULL	NULL	0	NULL	patient management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The customary telephone call between resident and attending physician benefited from the additional photographic data , and patient management resulted in a clear , concise , and unambiguous treatment plan .
	manualset3
145671	6	409378	5	NULL	NULL	0	NULL	treatment plan	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The customary telephone call between resident and attending physician benefited from the additional photographic data , and patient management resulted in a clear , concise , and unambiguous treatment plan .
	manualset3
145672	1	409379	5	NULL	NULL	0	NULL	cutaneous manifestations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cutaneous manifestations of parvovirus infection seem secondary to infection of the endothelium and epidermis .
	manualset3
145673	2	409379	5	NULL	NULL	0	NULL	parvovirus infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cutaneous manifestations of parvovirus infection seem secondary to infection of the endothelium and epidermis .
	manualset3
145674	3	409379	5	NULL	NULL	0	NULL	infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cutaneous manifestations of parvovirus infection seem secondary to infection of the endothelium and epidermis .
	manualset3
145675	4	409379	5	NULL	NULL	0	NULL	endothelium	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The cutaneous manifestations of parvovirus infection seem secondary to infection of the endothelium and epidermis .
	manualset3
145676	5	409379	5	NULL	NULL	0	NULL	epidermis	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The cutaneous manifestations of parvovirus infection seem secondary to infection of the endothelium and epidermis .
	manualset3
145677	1	409380	5	NULL	NULL	0	NULL	cyanobacterium	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The cyanobacterium produced inhibitory metabolites intracellularly at all stages of its growth cycle .
	manualset3
145678	2	409380	5	NULL	NULL	0	NULL	 inhibitory metabolites	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The cyanobacterium produced inhibitory metabolites intracellularly at all stages of its growth cycle .
	manualset3
145679	3	409380	5	NULL	NULL	0	NULL	stages	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The cyanobacterium produced inhibitory metabolites intracellularly at all stages of its growth cycle .
	manualset3
145680	4	409380	5	NULL	NULL	0	NULL	growth cycle 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cyanobacterium produced inhibitory metabolites intracellularly at all stages of its growth cycle .
	manualset3
145681	1	409381	5	NULL	NULL	0	NULL	cyanomethyl analog 3	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The cyanomethyl analog 3 was less active than 2 in all the test systems , except the inhibition of dihydrofolate reductase .
	manualset3
145682	2	409381	5	NULL	NULL	0	NULL	 cyanomethyl analog 2	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The cyanomethyl analog 3 was less active than 2 in all the test systems , except the inhibition of dihydrofolate reductase .
	manualset3
145683	3	409381	5	NULL	NULL	0	NULL	test systems	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cyanomethyl analog 3 was less active than 2 in all the test systems , except the inhibition of dihydrofolate reductase .
	manualset3
145684	4	409381	5	NULL	NULL	0	NULL	inhibition 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cyanomethyl analog 3 was less active than 2 in all the test systems , except the inhibition of dihydrofolate reductase .
	manualset3
145685	5	409381	5	NULL	NULL	0	NULL	dihydrofolate reductase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The cyanomethyl analog 3 was less active than 2 in all the test systems , except the inhibition of dihydrofolate reductase .
	manualset3
145686	1	409382	5	NULL	NULL	0	NULL	cysteine adducts 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The cysteine adducts arose through addition of glutathione to the thiirane ring .
	manualset3
145687	2	409382	5	NULL	NULL	0	NULL	glutathione 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The cysteine adducts arose through addition of glutathione to the thiirane ring .
	manualset3
145688	3	409382	5	NULL	NULL	0	NULL	thiirane ring	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The cysteine adducts arose through addition of glutathione to the thiirane ring .
	manualset3
145689	1	409383	5	NULL	NULL	0	NULL	cytogenetic locations	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytogenetic locations of the genes for protein C ( PROC ) , transition protein 1 ( TNP1 ) , intestinal alkaline phosphatase ( ALPI ) , engrailed ( EN1 ) , and human protointerleukin beta ( IL1B ) have been compared between cattle ( Bos taurus , BTA ) and sheep ( Ovis aries , OAR ) .
	manualset3
145690	2	409383	5	NULL	NULL	0	NULL	genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytogenetic locations of the genes for protein C ( PROC ) , transition protein 1 ( TNP1 ) , intestinal alkaline phosphatase ( ALPI ) , engrailed ( EN1 ) , and human protointerleukin beta ( IL1B ) have been compared between cattle ( Bos taurus , BTA ) and sheep ( Ovis aries , OAR ) .
	manualset3
145691	3	409383	5	NULL	NULL	0	NULL	protein C ( PROC )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytogenetic locations of the genes for protein C ( PROC ) , transition protein 1 ( TNP1 ) , intestinal alkaline phosphatase ( ALPI ) , engrailed ( EN1 ) , and human protointerleukin beta ( IL1B ) have been compared between cattle ( Bos taurus , BTA ) and sheep ( Ovis aries , OAR ) .
	manualset3
145692	4	409383	5	NULL	NULL	0	NULL	transition protein 1 ( TNP1 )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytogenetic locations of the genes for protein C ( PROC ) , transition protein 1 ( TNP1 ) , intestinal alkaline phosphatase ( ALPI ) , engrailed ( EN1 ) , and human protointerleukin beta ( IL1B ) have been compared between cattle ( Bos taurus , BTA ) and sheep ( Ovis aries , OAR ) .
	manualset3
145693	5	409383	5	NULL	NULL	0	NULL	intestinal alkaline phosphatase ( ALPI )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytogenetic locations of the genes for protein C ( PROC ) , transition protein 1 ( TNP1 ) , intestinal alkaline phosphatase ( ALPI ) , engrailed ( EN1 ) , and human protointerleukin beta ( IL1B ) have been compared between cattle ( Bos taurus , BTA ) and sheep ( Ovis aries , OAR ) .
	manualset3
145694	6	409383	5	NULL	NULL	0	NULL	engrailed ( EN1 )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytogenetic locations of the genes for protein C ( PROC ) , transition protein 1 ( TNP1 ) , intestinal alkaline phosphatase ( ALPI ) , engrailed ( EN1 ) , and human protointerleukin beta ( IL1B ) have been compared between cattle ( Bos taurus , BTA ) and sheep ( Ovis aries , OAR ) .
	manualset3
145695	7	409383	5	NULL	NULL	0	NULL	human protointerleukin beta ( IL1B )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytogenetic locations of the genes for protein C ( PROC ) , transition protein 1 ( TNP1 ) , intestinal alkaline phosphatase ( ALPI ) , engrailed ( EN1 ) , and human protointerleukin beta ( IL1B ) have been compared between cattle ( Bos taurus , BTA ) and sheep ( Ovis aries , OAR ) .
	manualset3
145696	8	409383	5	NULL	NULL	0	NULL	cattle ( Bos taurus , BTA )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytogenetic locations of the genes for protein C ( PROC ) , transition protein 1 ( TNP1 ) , intestinal alkaline phosphatase ( ALPI ) , engrailed ( EN1 ) , and human protointerleukin beta ( IL1B ) have been compared between cattle ( Bos taurus , BTA ) and sheep ( Ovis aries , OAR ) .
	manualset3
145697	9	409383	5	NULL	NULL	0	NULL	sheep ( Ovis aries , OAR )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytogenetic locations of the genes for protein C ( PROC ) , transition protein 1 ( TNP1 ) , intestinal alkaline phosphatase ( ALPI ) , engrailed ( EN1 ) , and human protointerleukin beta ( IL1B ) have been compared between cattle ( Bos taurus , BTA ) and sheep ( Ovis aries , OAR ) .
	manualset3
145698	1	409384	5	NULL	NULL	NULL	NULL	cytologic distinction	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The cytologic distinction from other benign and malignant breast lesions and its clinical significance are discussed .
	manualset3
145699	2	409384	5	NULL	NULL	0	NULL	benign breast lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytologic distinction from other benign and malignant breast lesions and its clinical significance are discussed .
	manualset3
145700	3	409384	5	NULL	NULL	0	NULL	malignant breast lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytologic distinction from other benign and malignant breast lesions and its clinical significance are discussed .
	manualset3
145701	4	409384	5	NULL	NULL	0	NULL	clinical significance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytologic distinction from other benign and malignant breast lesions and its clinical significance are discussed .
	manualset3
145702	1	409385	5	NULL	NULL	NULL	NULL	cytometric approach	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The cytometric approach permits one to detect , differentiate , and quantify cellular changes in these parasites resulting from drug treatment , in this case allopurinol , as well as demonstrate differences in drug susceptibility between promastigote forms .
	manualset3
145703	2	409385	5	NULL	NULL	0	NULL	one 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytometric approach permits one to detect , differentiate , and quantify cellular changes in these parasites resulting from drug treatment , in this case allopurinol , as well as demonstrate differences in drug susceptibility between promastigote forms .
	manualset3
145704	3	409385	5	NULL	NULL	NULL	NULL	cellular changes	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The cytometric approach permits one to detect , differentiate , and quantify cellular changes in these parasites resulting from drug treatment , in this case allopurinol , as well as demonstrate differences in drug susceptibility between promastigote forms .
	manualset3
145705	4	409385	5	NULL	NULL	0	NULL	parasites 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytometric approach permits one to detect , differentiate , and quantify cellular changes in these parasites resulting from drug treatment , in this case allopurinol , as well as demonstrate differences in drug susceptibility between promastigote forms .
	manualset3
145706	5	409385	5	NULL	NULL	0	NULL	drug treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytometric approach permits one to detect , differentiate , and quantify cellular changes in these parasites resulting from drug treatment , in this case allopurinol , as well as demonstrate differences in drug susceptibility between promastigote forms .
	manualset3
145707	6	409385	5	NULL	NULL	0	NULL	case 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytometric approach permits one to detect , differentiate , and quantify cellular changes in these parasites resulting from drug treatment , in this case allopurinol , as well as demonstrate differences in drug susceptibility between promastigote forms .
	manualset3
145708	7	409385	5	NULL	NULL	0	NULL	allopurinol 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytometric approach permits one to detect , differentiate , and quantify cellular changes in these parasites resulting from drug treatment , in this case allopurinol , as well as demonstrate differences in drug susceptibility between promastigote forms .
	manualset3
145709	8	409385	5	NULL	NULL	0	NULL	drug susceptibility 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytometric approach permits one to detect , differentiate , and quantify cellular changes in these parasites resulting from drug treatment , in this case allopurinol , as well as demonstrate differences in drug susceptibility between promastigote forms .
	manualset3
145710	9	409385	5	NULL	NULL	0	NULL	promastigote forms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytometric approach permits one to detect , differentiate , and quantify cellular changes in these parasites resulting from drug treatment , in this case allopurinol , as well as demonstrate differences in drug susceptibility between promastigote forms .
	manualset3
145711	1	409386	5	NULL	NULL	0	NULL	high-performance liquid chromatography ( HPLC ) - mass spectrometric ( MS ) method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple , fast and sensitive high-performance liquid chromatography ( HPLC ) - mass spectrometric ( MS ) method has been developed for simultaneous determination of amoxicillin and clavulanic acid in human plasma using terbutaline as internal standard .
	manualset3
145712	2	409386	5	NULL	NULL	0	NULL	determination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple , fast and sensitive high-performance liquid chromatography ( HPLC ) - mass spectrometric ( MS ) method has been developed for simultaneous determination of amoxicillin and clavulanic acid in human plasma using terbutaline as internal standard .
	manualset3
145713	3	409386	5	NULL	NULL	0	NULL	amoxicillin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple , fast and sensitive high-performance liquid chromatography ( HPLC ) - mass spectrometric ( MS ) method has been developed for simultaneous determination of amoxicillin and clavulanic acid in human plasma using terbutaline as internal standard .
	manualset3
145714	4	409386	5	NULL	NULL	0	NULL	clavulanic acid 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple , fast and sensitive high-performance liquid chromatography ( HPLC ) - mass spectrometric ( MS ) method has been developed for simultaneous determination of amoxicillin and clavulanic acid in human plasma using terbutaline as internal standard .
	manualset3
145715	5	409386	5	NULL	NULL	0	NULL	human plasma 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple , fast and sensitive high-performance liquid chromatography ( HPLC ) - mass spectrometric ( MS ) method has been developed for simultaneous determination of amoxicillin and clavulanic acid in human plasma using terbutaline as internal standard .
	manualset3
145716	6	409386	5	NULL	NULL	0	NULL	terbutaline 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple , fast and sensitive high-performance liquid chromatography ( HPLC ) - mass spectrometric ( MS ) method has been developed for simultaneous determination of amoxicillin and clavulanic acid in human plasma using terbutaline as internal standard .
	manualset3
145717	7	409386	5	NULL	NULL	0	NULL	internal standard	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple , fast and sensitive high-performance liquid chromatography ( HPLC ) - mass spectrometric ( MS ) method has been developed for simultaneous determination of amoxicillin and clavulanic acid in human plasma using terbutaline as internal standard .
	manualset3
145718	1	409387	5	NULL	NULL	0	NULL	cytoplasm 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytoplasm of the endothelial cells , especially in the arterioles , was segmentally thickened and contained numerous vesicles and vacuoles , some of which were HRP positive .
	manualset3
145719	2	409387	5	NULL	NULL	0	NULL	endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytoplasm of the endothelial cells , especially in the arterioles , was segmentally thickened and contained numerous vesicles and vacuoles , some of which were HRP positive .
	manualset3
145720	3	409387	5	NULL	NULL	0	NULL	arterioles 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytoplasm of the endothelial cells , especially in the arterioles , was segmentally thickened and contained numerous vesicles and vacuoles , some of which were HRP positive .
	manualset3
145721	4	409387	5	NULL	NULL	0	NULL	vesicles 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytoplasm of the endothelial cells , especially in the arterioles , was segmentally thickened and contained numerous vesicles and vacuoles , some of which were HRP positive .
	manualset3
145722	5	409387	5	NULL	NULL	0	NULL	vacuoles 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytoplasm of the endothelial cells , especially in the arterioles , was segmentally thickened and contained numerous vesicles and vacuoles , some of which were HRP positive .
	manualset3
145723	6	409387	5	NULL	NULL	0	NULL	HRP 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytoplasm of the endothelial cells , especially in the arterioles , was segmentally thickened and contained numerous vesicles and vacuoles , some of which were HRP positive .
	manualset3
145724	1	409388	5	NULL	NULL	0	NULL	cytoplasm 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytoplasm was characterized by the presence of alternately clear and dense sites .
	manualset3
145725	2	409388	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytoplasm was characterized by the presence of alternately clear and dense sites .
	manualset3
145726	3	409388	5	NULL	NULL	0	NULL	alternately clear and dense sites	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytoplasm was characterized by the presence of alternately clear and dense sites .
	manualset3
145727	1	409389	5	NULL	NULL	0	NULL	cytoplasmic catenins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytoplasmic catenins link the cell membrane-associated cadherins to the actin-based cytoskeleton .
	manualset3
145728	2	409389	5	NULL	NULL	0	NULL	cell membrane-associated cadherins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytoplasmic catenins link the cell membrane-associated cadherins to the actin-based cytoskeleton .
	manualset3
145729	3	409389	5	NULL	NULL	0	NULL	actin-based cytoskeleton	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytoplasmic catenins link the cell membrane-associated cadherins to the actin-based cytoskeleton .
	manualset3
145730	1	409390	5	NULL	NULL	0	NULL	cytoplasmic matrix	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytoplasmic matrix is of moderately low density .
	manualset3
145731	2	409390	5	NULL	NULL	0	NULL	density 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytoplasmic matrix is of moderately low density .
	manualset3
145732	1	409391	5	NULL	NULL	0	NULL	cytoplasmic membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytoplasmic membrane of E. coli AW1 .7 contained a higher proportion of saturated and cyclopropane fatty acids than that of E. coli GGG10 .
	manualset3
145733	2	409391	5	NULL	NULL	0	NULL	E. coli AW1 .7	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytoplasmic membrane of E. coli AW1 .7 contained a higher proportion of saturated and cyclopropane fatty acids than that of E. coli GGG10 .
	manualset3
145734	3	409391	5	NULL	NULL	0	NULL	proportion 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytoplasmic membrane of E. coli AW1 .7 contained a higher proportion of saturated and cyclopropane fatty acids than that of E. coli GGG10 .
	manualset3
145735	4	409391	5	NULL	NULL	0	NULL	saturated fatty acids	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytoplasmic membrane of E. coli AW1 .7 contained a higher proportion of saturated and cyclopropane fatty acids than that of E. coli GGG10 .
	manualset3
145736	5	409391	5	NULL	NULL	0	NULL	cyclopropane fatty acids 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytoplasmic membrane of E. coli AW1 .7 contained a higher proportion of saturated and cyclopropane fatty acids than that of E. coli GGG10 .
	manualset3
145737	6	409391	5	NULL	NULL	0	NULL	E. coli GGG10	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytoplasmic membrane of E. coli AW1 .7 contained a higher proportion of saturated and cyclopropane fatty acids than that of E. coli GGG10 .
	manualset3
145738	1	409392	5	NULL	NULL	0	NULL	cytoprotective activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytoprotective activity of BHA was also compared with that of the structurally unrelated antioxidant ebselen .
	manualset3
145739	2	409392	5	NULL	NULL	0	NULL	BHA 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytoprotective activity of BHA was also compared with that of the structurally unrelated antioxidant ebselen .
	manualset3
145740	3	409392	5	NULL	NULL	0	NULL	antioxidant ebselen	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytoprotective activity of BHA was also compared with that of the structurally unrelated antioxidant ebselen .
	manualset3
145741	1	409393	5	NULL	NULL	0	NULL	damage 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The damage can be lowered by the application of a mixture of antioxidants , the most important are vitamin C , A , E , glutathione , selenium , carnosine , eventually bioflavonoids and ginkgo biloba .
	manualset3
145742	2	409393	5	NULL	NULL	0	NULL	application 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The damage can be lowered by the application of a mixture of antioxidants , the most important are vitamin C , A , E , glutathione , selenium , carnosine , eventually bioflavonoids and ginkgo biloba .
	manualset3
145743	3	409393	5	NULL	NULL	0	NULL	mixture 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The damage can be lowered by the application of a mixture of antioxidants , the most important are vitamin C , A , E , glutathione , selenium , carnosine , eventually bioflavonoids and ginkgo biloba .
	manualset3
145744	4	409393	5	NULL	NULL	0	NULL	antioxidants 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The damage can be lowered by the application of a mixture of antioxidants , the most important are vitamin C , A , E , glutathione , selenium , carnosine , eventually bioflavonoids and ginkgo biloba .
	manualset3
145745	5	409393	5	NULL	NULL	0	NULL	vitamin C	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The damage can be lowered by the application of a mixture of antioxidants , the most important are vitamin C , A , E , glutathione , selenium , carnosine , eventually bioflavonoids and ginkgo biloba .
	manualset3
145746	6	409393	5	NULL	NULL	0	NULL	vitamin A	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The damage can be lowered by the application of a mixture of antioxidants , the most important are vitamin C , A , E , glutathione , selenium , carnosine , eventually bioflavonoids and ginkgo biloba .
	manualset3
145747	7	409393	5	NULL	NULL	0	NULL	vitamin E	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The damage can be lowered by the application of a mixture of antioxidants , the most important are vitamin C , A , E , glutathione , selenium , carnosine , eventually bioflavonoids and ginkgo biloba .
	manualset3
145748	8	409393	5	NULL	NULL	0	NULL	glutathione 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The damage can be lowered by the application of a mixture of antioxidants , the most important are vitamin C , A , E , glutathione , selenium , carnosine , eventually bioflavonoids and ginkgo biloba .
	manualset3
145749	9	409393	5	NULL	NULL	0	NULL	selenium 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The damage can be lowered by the application of a mixture of antioxidants , the most important are vitamin C , A , E , glutathione , selenium , carnosine , eventually bioflavonoids and ginkgo biloba .
	manualset3
145750	10	409393	5	NULL	NULL	0	NULL	carnosine 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The damage can be lowered by the application of a mixture of antioxidants , the most important are vitamin C , A , E , glutathione , selenium , carnosine , eventually bioflavonoids and ginkgo biloba .
	manualset3
145751	11	409393	5	NULL	NULL	0	NULL	bioflavonoids 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The damage can be lowered by the application of a mixture of antioxidants , the most important are vitamin C , A , E , glutathione , selenium , carnosine , eventually bioflavonoids and ginkgo biloba .
	manualset3
145752	12	409393	5	NULL	NULL	0	NULL	ginkgo biloba	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The damage can be lowered by the application of a mixture of antioxidants , the most important are vitamin C , A , E , glutathione , selenium , carnosine , eventually bioflavonoids and ginkgo biloba .
	manualset3
145753	1	409394	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data also show that the reason why ADM does not inhibit osteoclast activity or formation is related to the fact that RANKL decreases ADM receptor signaling through the adenylate cyclase-cyclic AMP pathway .
	manualset3
145754	2	409394	5	NULL	NULL	0	NULL	reason 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data also show that the reason why ADM does not inhibit osteoclast activity or formation is related to the fact that RANKL decreases ADM receptor signaling through the adenylate cyclase-cyclic AMP pathway .
	manualset3
145755	3	409394	5	NULL	NULL	0	NULL	ADM 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The data also show that the reason why ADM does not inhibit osteoclast activity or formation is related to the fact that RANKL decreases ADM receptor signaling through the adenylate cyclase-cyclic AMP pathway .
	manualset3
145756	4	409394	5	NULL	NULL	0	NULL	osteoclast activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data also show that the reason why ADM does not inhibit osteoclast activity or formation is related to the fact that RANKL decreases ADM receptor signaling through the adenylate cyclase-cyclic AMP pathway .
	manualset3
145757	5	409394	5	NULL	NULL	0	NULL	osteoclast formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data also show that the reason why ADM does not inhibit osteoclast activity or formation is related to the fact that RANKL decreases ADM receptor signaling through the adenylate cyclase-cyclic AMP pathway .
	manualset3
145758	6	409394	5	NULL	NULL	0	NULL	RANKL 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The data also show that the reason why ADM does not inhibit osteoclast activity or formation is related to the fact that RANKL decreases ADM receptor signaling through the adenylate cyclase-cyclic AMP pathway .
	manualset3
145759	7	409394	5	NULL	NULL	0	NULL	ADM receptor signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data also show that the reason why ADM does not inhibit osteoclast activity or formation is related to the fact that RANKL decreases ADM receptor signaling through the adenylate cyclase-cyclic AMP pathway .
	manualset3
145760	8	409394	5	NULL	NULL	0	NULL	adenylate cyclase-cyclic AMP pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data also show that the reason why ADM does not inhibit osteoclast activity or formation is related to the fact that RANKL decreases ADM receptor signaling through the adenylate cyclase-cyclic AMP pathway .
	manualset3
145761	1	409395	5	NULL	NULL	0	NULL	reverse phase high performance liquid chromatography ( HPLC ) method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple , precise , accurate and validated , acetonitrile-free , reverse phase high performance liquid chromatography ( HPLC ) method is developed for the determination of melamine in dry and liquid infant formula .
	manualset3
145762	2	409395	5	NULL	NULL	0	NULL	determination 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple , precise , accurate and validated , acetonitrile-free , reverse phase high performance liquid chromatography ( HPLC ) method is developed for the determination of melamine in dry and liquid infant formula .
	manualset3
145763	3	409395	5	NULL	NULL	0	NULL	melamine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple , precise , accurate and validated , acetonitrile-free , reverse phase high performance liquid chromatography ( HPLC ) method is developed for the determination of melamine in dry and liquid infant formula .
	manualset3
145764	4	409395	5	NULL	NULL	0	NULL	dry infant formula	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple , precise , accurate and validated , acetonitrile-free , reverse phase high performance liquid chromatography ( HPLC ) method is developed for the determination of melamine in dry and liquid infant formula .
	manualset3
145765	5	409395	5	NULL	NULL	0	NULL	liquid infant formula	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple , precise , accurate and validated , acetonitrile-free , reverse phase high performance liquid chromatography ( HPLC ) method is developed for the determination of melamine in dry and liquid infant formula .
	manualset3
145766	1	409396	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data appear to be compatible with the suggestion that the nucleotides may bind to sites in the membranes and subsequently induce conformational changes in membrane components , resulting in a decreased affinity of gonadotropin receptors .
	manualset3
145767	2	409396	5	NULL	NULL	0	NULL	suggestion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data appear to be compatible with the suggestion that the nucleotides may bind to sites in the membranes and subsequently induce conformational changes in membrane components , resulting in a decreased affinity of gonadotropin receptors .
	manualset3
145768	3	409396	5	NULL	NULL	0	NULL	nucleotides 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The data appear to be compatible with the suggestion that the nucleotides may bind to sites in the membranes and subsequently induce conformational changes in membrane components , resulting in a decreased affinity of gonadotropin receptors .
	manualset3
145769	4	409396	5	NULL	NULL	0	NULL	sites in the membranes 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The data appear to be compatible with the suggestion that the nucleotides may bind to sites in the membranes and subsequently induce conformational changes in membrane components , resulting in a decreased affinity of gonadotropin receptors .
	manualset3
145770	5	409396	5	NULL	NULL	0	NULL	conformational changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data appear to be compatible with the suggestion that the nucleotides may bind to sites in the membranes and subsequently induce conformational changes in membrane components , resulting in a decreased affinity of gonadotropin receptors .
	manualset3
145771	6	409396	5	NULL	NULL	0	NULL	membrane components	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The data appear to be compatible with the suggestion that the nucleotides may bind to sites in the membranes and subsequently induce conformational changes in membrane components , resulting in a decreased affinity of gonadotropin receptors .
	manualset3
145772	7	409396	5	NULL	NULL	0	NULL	decreased affinity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data appear to be compatible with the suggestion that the nucleotides may bind to sites in the membranes and subsequently induce conformational changes in membrane components , resulting in a decreased affinity of gonadotropin receptors .
	manualset3
145773	8	409396	5	NULL	NULL	0	NULL	gonadotropin receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The data appear to be compatible with the suggestion that the nucleotides may bind to sites in the membranes and subsequently induce conformational changes in membrane components , resulting in a decreased affinity of gonadotropin receptors .
	manualset3
145774	1	409397	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data are also interpreted in terms of `` reducing charge '' , the mole fraction of coenzyme in the reduced form .
	manualset3
145775	2	409397	5	NULL	NULL	0	NULL	reducing charge	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data are also interpreted in terms of `` reducing charge '' , the mole fraction of coenzyme in the reduced form .
	manualset3
145776	3	409397	5	NULL	NULL	0	NULL	mole fraction	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data are also interpreted in terms of `` reducing charge '' , the mole fraction of coenzyme in the reduced form .
	manualset3
145777	4	409397	5	NULL	NULL	0	NULL	coenzyme 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The data are also interpreted in terms of `` reducing charge '' , the mole fraction of coenzyme in the reduced form .
	manualset3
145778	5	409397	5	NULL	NULL	0	NULL	reduced form	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data are also interpreted in terms of `` reducing charge '' , the mole fraction of coenzyme in the reduced form .
	manualset3
145779	1	409398	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data are consistent with a mutational mechanism that requires transcription of the rearranged target V ( D ) J gene which appears to result in the generation of a positively skewed asymmetrical distribution of somatic mutations .
	manualset3
145780	2	409398	5	NULL	NULL	0	NULL	mutational mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data are consistent with a mutational mechanism that requires transcription of the rearranged target V ( D ) J gene which appears to result in the generation of a positively skewed asymmetrical distribution of somatic mutations .
	manualset3
145781	3	409398	5	NULL	NULL	0	NULL	transcription 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data are consistent with a mutational mechanism that requires transcription of the rearranged target V ( D ) J gene which appears to result in the generation of a positively skewed asymmetrical distribution of somatic mutations .
	manualset3
145782	4	409398	5	NULL	NULL	0	NULL	rearranged target V ( D ) J gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The data are consistent with a mutational mechanism that requires transcription of the rearranged target V ( D ) J gene which appears to result in the generation of a positively skewed asymmetrical distribution of somatic mutations .
	manualset3
145783	5	409398	5	NULL	NULL	0	NULL	result 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data are consistent with a mutational mechanism that requires transcription of the rearranged target V ( D ) J gene which appears to result in the generation of a positively skewed asymmetrical distribution of somatic mutations .
	manualset3
145784	6	409398	5	NULL	NULL	0	NULL	generation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data are consistent with a mutational mechanism that requires transcription of the rearranged target V ( D ) J gene which appears to result in the generation of a positively skewed asymmetrical distribution of somatic mutations .
	manualset3
145785	7	409398	5	NULL	NULL	0	NULL	positively skewed asymmetrical distribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data are consistent with a mutational mechanism that requires transcription of the rearranged target V ( D ) J gene which appears to result in the generation of a positively skewed asymmetrical distribution of somatic mutations .
	manualset3
145786	8	409398	5	NULL	NULL	0	NULL	somatic mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data are consistent with a mutational mechanism that requires transcription of the rearranged target V ( D ) J gene which appears to result in the generation of a positively skewed asymmetrical distribution of somatic mutations .
	manualset3
145787	1	409399	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data are consistent with the idea that the overall conformation of T antigen is important for transactivation and that mutations in other regions that reduce or eliminate transactivation do so by altering the conformation or orientation of the N-terminal region so that its ability to interact with various targets is diminished or abolished .
	manualset3
145788	2	409399	5	NULL	NULL	0	NULL	idea 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data are consistent with the idea that the overall conformation of T antigen is important for transactivation and that mutations in other regions that reduce or eliminate transactivation do so by altering the conformation or orientation of the N-terminal region so that its ability to interact with various targets is diminished or abolished .
	manualset3
145789	3	409399	5	NULL	NULL	0	NULL	conformation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data are consistent with the idea that the overall conformation of T antigen is important for transactivation and that mutations in other regions that reduce or eliminate transactivation do so by altering the conformation or orientation of the N-terminal region so that its ability to interact with various targets is diminished or abolished .
	manualset3
145790	4	409399	5	NULL	NULL	0	NULL	T antigen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The data are consistent with the idea that the overall conformation of T antigen is important for transactivation and that mutations in other regions that reduce or eliminate transactivation do so by altering the conformation or orientation of the N-terminal region so that its ability to interact with various targets is diminished or abolished .
	manualset3
145791	5	409399	5	NULL	NULL	0	NULL	transactivation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data are consistent with the idea that the overall conformation of T antigen is important for transactivation and that mutations in other regions that reduce or eliminate transactivation do so by altering the conformation or orientation of the N-terminal region so that its ability to interact with various targets is diminished or abolished .
	manualset3
145792	6	409399	5	NULL	NULL	0	NULL	mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data are consistent with the idea that the overall conformation of T antigen is important for transactivation and that mutations in other regions that reduce or eliminate transactivation do so by altering the conformation or orientation of the N-terminal region so that its ability to interact with various targets is diminished or abolished .
	manualset3
145793	7	409399	5	NULL	NULL	0	NULL	regions 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data are consistent with the idea that the overall conformation of T antigen is important for transactivation and that mutations in other regions that reduce or eliminate transactivation do so by altering the conformation or orientation of the N-terminal region so that its ability to interact with various targets is diminished or abolished .
	manualset3
145794	8	409399	5	NULL	NULL	0	NULL	transactivation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data are consistent with the idea that the overall conformation of T antigen is important for transactivation and that mutations in other regions that reduce or eliminate transactivation do so by altering the conformation or orientation of the N-terminal region so that its ability to interact with various targets is diminished or abolished .
	manualset3
145795	9	409399	5	NULL	NULL	0	NULL	conformation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data are consistent with the idea that the overall conformation of T antigen is important for transactivation and that mutations in other regions that reduce or eliminate transactivation do so by altering the conformation or orientation of the N-terminal region so that its ability to interact with various targets is diminished or abolished .
	manualset3
145796	10	409399	5	NULL	NULL	0	NULL	orientation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data are consistent with the idea that the overall conformation of T antigen is important for transactivation and that mutations in other regions that reduce or eliminate transactivation do so by altering the conformation or orientation of the N-terminal region so that its ability to interact with various targets is diminished or abolished .
	manualset3
145797	11	409399	5	NULL	NULL	0	NULL	N-terminal region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The data are consistent with the idea that the overall conformation of T antigen is important for transactivation and that mutations in other regions that reduce or eliminate transactivation do so by altering the conformation or orientation of the N-terminal region so that its ability to interact with various targets is diminished or abolished .
	manualset3
145798	12	409399	5	NULL	NULL	0	NULL	ability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data are consistent with the idea that the overall conformation of T antigen is important for transactivation and that mutations in other regions that reduce or eliminate transactivation do so by altering the conformation or orientation of the N-terminal region so that its ability to interact with various targets is diminished or abolished .
	manualset3
145799	13	409399	5	NULL	NULL	0	NULL	interact 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data are consistent with the idea that the overall conformation of T antigen is important for transactivation and that mutations in other regions that reduce or eliminate transactivation do so by altering the conformation or orientation of the N-terminal region so that its ability to interact with various targets is diminished or abolished .
	manualset3
145800	14	409399	5	NULL	NULL	NULL	NULL	targets 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The data are consistent with the idea that the overall conformation of T antigen is important for transactivation and that mutations in other regions that reduce or eliminate transactivation do so by altering the conformation or orientation of the N-terminal region so that its ability to interact with various targets is diminished or abolished .
	manualset3
145801	1	409400	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data challenge the notion that aGVHD is purely a Th1-type cytokine-driven response , high-lighting a novel and highly significant link between the Th2-type cytokine IL-13 and aGVHD .
	manualset3
145802	2	409400	5	NULL	NULL	0	NULL	notion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data challenge the notion that aGVHD is purely a Th1-type cytokine-driven response , high-lighting a novel and highly significant link between the Th2-type cytokine IL-13 and aGVHD .
	manualset3
145803	3	409400	5	NULL	NULL	0	NULL	aGVHD 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The data challenge the notion that aGVHD is purely a Th1-type cytokine-driven response , high-lighting a novel and highly significant link between the Th2-type cytokine IL-13 and aGVHD .
	manualset3
145804	4	409400	5	NULL	NULL	0	NULL	Th1-type cytokine-driven response 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data challenge the notion that aGVHD is purely a Th1-type cytokine-driven response , high-lighting a novel and highly significant link between the Th2-type cytokine IL-13 and aGVHD .
	manualset3
145805	5	409400	5	NULL	NULL	0	NULL	 significant link	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data challenge the notion that aGVHD is purely a Th1-type cytokine-driven response , high-lighting a novel and highly significant link between the Th2-type cytokine IL-13 and aGVHD .
	manualset3
145806	6	409400	5	NULL	NULL	0	NULL	Th2-type cytokine IL-13	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The data challenge the notion that aGVHD is purely a Th1-type cytokine-driven response , high-lighting a novel and highly significant link between the Th2-type cytokine IL-13 and aGVHD .
	manualset3
145807	7	409400	5	NULL	NULL	0	NULL	aGVHD 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The data challenge the notion that aGVHD is purely a Th1-type cytokine-driven response , high-lighting a novel and highly significant link between the Th2-type cytokine IL-13 and aGVHD .
	manualset3
145808	1	409401	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data clearly showed that reliability was not influenced by the objectivity or subjectivity of the test measure .
	manualset3
145809	2	409401	5	NULL	NULL	0	NULL	reliability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data clearly showed that reliability was not influenced by the objectivity or subjectivity of the test measure .
	manualset3
145810	3	409401	5	NULL	NULL	0	NULL	objectivity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data clearly showed that reliability was not influenced by the objectivity or subjectivity of the test measure .
	manualset3
145811	4	409401	5	NULL	NULL	0	NULL	subjectivity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data clearly showed that reliability was not influenced by the objectivity or subjectivity of the test measure .
	manualset3
145812	5	409401	5	NULL	NULL	0	NULL	test measure	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The data clearly showed that reliability was not influenced by the objectivity or subjectivity of the test measure .
	manualset3
145813	1	409402	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data concerning the serum levels of carnitine , in patients with ESRD on continuous ambulatory peritoneal dialysis ( CAPD ) are contradictory , but most of them support that they are rather normal .
	manualset3
145814	2	409402	5	NULL	NULL	0	NULL	serum levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data concerning the serum levels of carnitine , in patients with ESRD on continuous ambulatory peritoneal dialysis ( CAPD ) are contradictory , but most of them support that they are rather normal .
	manualset3
145815	3	409402	5	NULL	NULL	0	NULL	carnitine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The data concerning the serum levels of carnitine , in patients with ESRD on continuous ambulatory peritoneal dialysis ( CAPD ) are contradictory , but most of them support that they are rather normal .
	manualset3
145816	4	409402	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The data concerning the serum levels of carnitine , in patients with ESRD on continuous ambulatory peritoneal dialysis ( CAPD ) are contradictory , but most of them support that they are rather normal .
	manualset3
145817	5	409402	5	NULL	NULL	0	NULL	ESRD 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The data concerning the serum levels of carnitine , in patients with ESRD on continuous ambulatory peritoneal dialysis ( CAPD ) are contradictory , but most of them support that they are rather normal .
	manualset3
145818	6	409402	5	NULL	NULL	0	NULL	continuous ambulatory peritoneal dialysis ( CAPD )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The data concerning the serum levels of carnitine , in patients with ESRD on continuous ambulatory peritoneal dialysis ( CAPD ) are contradictory , but most of them support that they are rather normal .
	manualset3
145819	1	409403	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data demonstrate that exposure to SO2 may reduce the chemotactic activity of AM and BM .
	manualset3
145820	2	409403	5	NULL	NULL	0	NULL	exposure 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data demonstrate that exposure to SO2 may reduce the chemotactic activity of AM and BM .
	manualset3
145821	3	409403	5	NULL	NULL	0	NULL	SO2	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The data demonstrate that exposure to SO2 may reduce the chemotactic activity of AM and BM .
	manualset3
145822	4	409403	5	NULL	NULL	0	NULL	chemotactic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data demonstrate that exposure to SO2 may reduce the chemotactic activity of AM and BM .
	manualset3
145823	5	409403	5	NULL	NULL	0	NULL	AM 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The data demonstrate that exposure to SO2 may reduce the chemotactic activity of AM and BM .
	manualset3
145824	6	409403	5	NULL	NULL	0	NULL	BM 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The data demonstrate that exposure to SO2 may reduce the chemotactic activity of AM and BM .
	manualset3
145825	1	409404	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data demonstrated that approximately 149 genes represented were positively regulated by T3 , including fibrinogen , transferrin , fibronectin ( FN ) , androgen receptor ( AR ) - associated protein ( ARA70 ) , and dehydroepiandrosterone sulfotransferase family 1A member 2 ( SULT2A1 ) .
	manualset3
145826	2	409404	5	NULL	NULL	0	NULL	149 genes	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The data demonstrated that approximately 149 genes represented were positively regulated by T3 , including fibrinogen , transferrin , fibronectin ( FN ) , androgen receptor ( AR ) - associated protein ( ARA70 ) , and dehydroepiandrosterone sulfotransferase family 1A member 2 ( SULT2A1 ) .
	manualset3
145827	3	409404	5	NULL	NULL	0	NULL	T3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The data demonstrated that approximately 149 genes represented were positively regulated by T3 , including fibrinogen , transferrin , fibronectin ( FN ) , androgen receptor ( AR ) - associated protein ( ARA70 ) , and dehydroepiandrosterone sulfotransferase family 1A member 2 ( SULT2A1 ) .
	manualset3
145828	4	409404	5	NULL	NULL	0	NULL	fibrinogen 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The data demonstrated that approximately 149 genes represented were positively regulated by T3 , including fibrinogen , transferrin , fibronectin ( FN ) , androgen receptor ( AR ) - associated protein ( ARA70 ) , and dehydroepiandrosterone sulfotransferase family 1A member 2 ( SULT2A1 ) .
	manualset3
145829	5	409404	5	NULL	NULL	0	NULL	transferrin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The data demonstrated that approximately 149 genes represented were positively regulated by T3 , including fibrinogen , transferrin , fibronectin ( FN ) , androgen receptor ( AR ) - associated protein ( ARA70 ) , and dehydroepiandrosterone sulfotransferase family 1A member 2 ( SULT2A1 ) .
	manualset3
145830	6	409404	5	NULL	NULL	0	NULL	fibronectin ( FN )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The data demonstrated that approximately 149 genes represented were positively regulated by T3 , including fibrinogen , transferrin , fibronectin ( FN ) , androgen receptor ( AR ) - associated protein ( ARA70 ) , and dehydroepiandrosterone sulfotransferase family 1A member 2 ( SULT2A1 ) .
	manualset3
145831	7	409404	5	NULL	NULL	0	NULL	androgen receptor ( AR ) - associated protein ( ARA70 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The data demonstrated that approximately 149 genes represented were positively regulated by T3 , including fibrinogen , transferrin , fibronectin ( FN ) , androgen receptor ( AR ) - associated protein ( ARA70 ) , and dehydroepiandrosterone sulfotransferase family 1A member 2 ( SULT2A1 ) .
	manualset3
145832	8	409404	5	NULL	NULL	0	NULL	dehydroepiandrosterone sulfotransferase family 1A member 2 ( SULT2A1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The data demonstrated that approximately 149 genes represented were positively regulated by T3 , including fibrinogen , transferrin , fibronectin ( FN ) , androgen receptor ( AR ) - associated protein ( ARA70 ) , and dehydroepiandrosterone sulfotransferase family 1A member 2 ( SULT2A1 ) .
	manualset3
145833	1	409405	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data did not conform to the subscale structure during factor analysis .
	manualset3
145834	2	409405	5	NULL	NULL	0	NULL	subscale structure 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data did not conform to the subscale structure during factor analysis .
	manualset3
145835	3	409405	5	NULL	NULL	0	NULL	factor analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data did not conform to the subscale structure during factor analysis .
	manualset3
145836	1	409406	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data do show that while it is very important to always be aware of alternative explanations for test results , the likelihood of external contamination confounding the interpretation of hair tests can be reduced to manageable proportions .
	manualset3
145837	2	409406	5	NULL	NULL	0	NULL	alternative explanations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data do show that while it is very important to always be aware of alternative explanations for test results , the likelihood of external contamination confounding the interpretation of hair tests can be reduced to manageable proportions .
	manualset3
145838	3	409406	5	NULL	NULL	0	NULL	test results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data do show that while it is very important to always be aware of alternative explanations for test results , the likelihood of external contamination confounding the interpretation of hair tests can be reduced to manageable proportions .
	manualset3
145839	4	409406	5	NULL	NULL	0	NULL	external contamination	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data do show that while it is very important to always be aware of alternative explanations for test results , the likelihood of external contamination confounding the interpretation of hair tests can be reduced to manageable proportions .
	manualset3
145840	5	409406	5	NULL	NULL	0	NULL	interpretation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data do show that while it is very important to always be aware of alternative explanations for test results , the likelihood of external contamination confounding the interpretation of hair tests can be reduced to manageable proportions .
	manualset3
145841	6	409406	5	NULL	NULL	0	NULL	hair tests	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data do show that while it is very important to always be aware of alternative explanations for test results , the likelihood of external contamination confounding the interpretation of hair tests can be reduced to manageable proportions .
	manualset3
145842	7	409406	5	NULL	NULL	0	NULL	manageable proportions	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The data do show that while it is very important to always be aware of alternative explanations for test results , the likelihood of external contamination confounding the interpretation of hair tests can be reduced to manageable proportions .
	manualset3
145843	1	409407	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data for the cones made with both test objects are adequately described by one and the same form of the stationary state equation derived by Hecht for the photoreceptor system .
	manualset3
145844	2	409407	5	NULL	NULL	0	NULL	cones 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The data for the cones made with both test objects are adequately described by one and the same form of the stationary state equation derived by Hecht for the photoreceptor system .
	manualset3
145845	3	409407	5	NULL	NULL	0	NULL	test objects	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data for the cones made with both test objects are adequately described by one and the same form of the stationary state equation derived by Hecht for the photoreceptor system .
	manualset3
145846	4	409407	5	NULL	NULL	0	NULL	one 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The data for the cones made with both test objects are adequately described by one and the same form of the stationary state equation derived by Hecht for the photoreceptor system .
	manualset3
145847	5	409407	5	NULL	NULL	0	NULL	stationary state equation	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The data for the cones made with both test objects are adequately described by one and the same form of the stationary state equation derived by Hecht for the photoreceptor system .
	manualset3
145848	6	409407	5	NULL	NULL	0	NULL	Hecht 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The data for the cones made with both test objects are adequately described by one and the same form of the stationary state equation derived by Hecht for the photoreceptor system .
	manualset3
145849	7	409407	5	NULL	NULL	0	NULL	photoreceptor system	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data for the cones made with both test objects are adequately described by one and the same form of the stationary state equation derived by Hecht for the photoreceptor system .
	manualset3
145850	1	409408	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data from stress conditions and their ratios ( trait measured under stress condition/trait measured under well water condition ) or differences ( trait measured under stress condition minus trait measured under well water condition ) were used for QTL analysis .
	manualset3
145851	2	409408	5	NULL	NULL	0	NULL	stress conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The data from stress conditions and their ratios ( trait measured under stress condition/trait measured under well water condition ) or differences ( trait measured under stress condition minus trait measured under well water condition ) were used for QTL analysis .
	manualset3
145852	3	409408	5	NULL	NULL	0	NULL	ratios 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data from stress conditions and their ratios ( trait measured under stress condition/trait measured under well water condition ) or differences ( trait measured under stress condition minus trait measured under well water condition ) were used for QTL analysis .
	manualset3
145853	4	409408	5	NULL	NULL	0	NULL	trait 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data from stress conditions and their ratios ( trait measured under stress condition/trait measured under well water condition ) or differences ( trait measured under stress condition minus trait measured under well water condition ) were used for QTL analysis .
	manualset3
145854	5	409408	5	NULL	NULL	0	NULL	stress condition/trait measured	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The data from stress conditions and their ratios ( trait measured under stress condition/trait measured under well water condition ) or differences ( trait measured under stress condition minus trait measured under well water condition ) were used for QTL analysis .
	manualset3
145855	6	409408	5	NULL	NULL	0	NULL	well water condition	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The data from stress conditions and their ratios ( trait measured under stress condition/trait measured under well water condition ) or differences ( trait measured under stress condition minus trait measured under well water condition ) were used for QTL analysis .
	manualset3
145856	7	409408	5	NULL	NULL	0	NULL	differences 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data from stress conditions and their ratios ( trait measured under stress condition/trait measured under well water condition ) or differences ( trait measured under stress condition minus trait measured under well water condition ) were used for QTL analysis .
	manualset3
145857	8	409408	5	NULL	NULL	0	NULL	trait 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data from stress conditions and their ratios ( trait measured under stress condition/trait measured under well water condition ) or differences ( trait measured under stress condition minus trait measured under well water condition ) were used for QTL analysis .
	manualset3
145858	9	409408	5	NULL	NULL	0	NULL	stress condition	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The data from stress conditions and their ratios ( trait measured under stress condition/trait measured under well water condition ) or differences ( trait measured under stress condition minus trait measured under well water condition ) were used for QTL analysis .
	manualset3
145859	10	409408	5	NULL	NULL	0	NULL	trait 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data from stress conditions and their ratios ( trait measured under stress condition/trait measured under well water condition ) or differences ( trait measured under stress condition minus trait measured under well water condition ) were used for QTL analysis .
	manualset3
145860	11	409408	5	NULL	NULL	0	NULL	well water condition	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The data from stress conditions and their ratios ( trait measured under stress condition/trait measured under well water condition ) or differences ( trait measured under stress condition minus trait measured under well water condition ) were used for QTL analysis .
	manualset3
145861	12	409408	5	NULL	NULL	0	NULL	QTL analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data from stress conditions and their ratios ( trait measured under stress condition/trait measured under well water condition ) or differences ( trait measured under stress condition minus trait measured under well water condition ) were used for QTL analysis .
	manualset3
145862	1	409409	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data further indicate that sarcomas in animals treated i.p. with acemannan at the time of tumor cell implantation were infiltrated by immune system cells , became necrotic , and regressed .
	manualset3
145863	2	409409	5	NULL	NULL	0	NULL	sarcomas 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The data further indicate that sarcomas in animals treated i.p. with acemannan at the time of tumor cell implantation were infiltrated by immune system cells , became necrotic , and regressed .
	manualset3
145864	3	409409	5	NULL	NULL	0	NULL	animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The data further indicate that sarcomas in animals treated i.p. with acemannan at the time of tumor cell implantation were infiltrated by immune system cells , became necrotic , and regressed .
	manualset3
145865	4	409409	5	NULL	NULL	0	NULL	acemannan 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The data further indicate that sarcomas in animals treated i.p. with acemannan at the time of tumor cell implantation were infiltrated by immune system cells , became necrotic , and regressed .
	manualset3
145866	5	409409	5	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The data further indicate that sarcomas in animals treated i.p. with acemannan at the time of tumor cell implantation were infiltrated by immune system cells , became necrotic , and regressed .
	manualset3
145867	6	409409	5	NULL	NULL	NULL	NULL	tumor cell implantation	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The data further indicate that sarcomas in animals treated i.p. with acemannan at the time of tumor cell implantation were infiltrated by immune system cells , became necrotic , and regressed .
	manualset3
145868	7	409409	5	NULL	NULL	0	NULL	immune system cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The data further indicate that sarcomas in animals treated i.p. with acemannan at the time of tumor cell implantation were infiltrated by immune system cells , became necrotic , and regressed .
	manualset3
145869	1	409410	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data here reported suggest that the growth capability of NK cell progenitors is under the control of the thymus .
	manualset3
145870	2	409410	5	NULL	NULL	0	NULL	growth capability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data here reported suggest that the growth capability of NK cell progenitors is under the control of the thymus .
	manualset3
145871	3	409410	5	NULL	NULL	0	NULL	NK cell progenitors	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The data here reported suggest that the growth capability of NK cell progenitors is under the control of the thymus .
	manualset3
145872	4	409410	5	NULL	NULL	0	NULL	control 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data here reported suggest that the growth capability of NK cell progenitors is under the control of the thymus .
	manualset3
145873	5	409410	5	NULL	NULL	0	NULL	thymus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The data here reported suggest that the growth capability of NK cell progenitors is under the control of the thymus .
	manualset3
145874	1	409411	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data indicate that DEHP , in clinically relevant concentrations , can impair the electrical and mechanical behavior of a cardiac cell network .
	manualset3
145875	2	409411	5	NULL	NULL	0	NULL	DEHP 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The data indicate that DEHP , in clinically relevant concentrations , can impair the electrical and mechanical behavior of a cardiac cell network .
	manualset3
145876	3	409411	5	NULL	NULL	0	NULL	clinically relevant concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data indicate that DEHP , in clinically relevant concentrations , can impair the electrical and mechanical behavior of a cardiac cell network .
	manualset3
145877	4	409411	5	NULL	NULL	0	NULL	electrical behavior 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data indicate that DEHP , in clinically relevant concentrations , can impair the electrical and mechanical behavior of a cardiac cell network .
	manualset3
145878	5	409411	5	NULL	NULL	0	NULL	mechanical behavior 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data indicate that DEHP , in clinically relevant concentrations , can impair the electrical and mechanical behavior of a cardiac cell network .
	manualset3
145879	6	409411	5	NULL	NULL	0	NULL	cardiac cell network	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The data indicate that DEHP , in clinically relevant concentrations , can impair the electrical and mechanical behavior of a cardiac cell network .
	manualset3
145880	1	409412	5	NULL	NULL	0	NULL	 gas chromatographic method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple and quick gas chromatographic method for the determination of propham and chlorpropham in potatoes .
	manualset3
145881	2	409412	5	NULL	NULL	0	NULL	determination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple and quick gas chromatographic method for the determination of propham and chlorpropham in potatoes .
	manualset3
145882	3	409412	5	NULL	NULL	0	NULL	propham 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple and quick gas chromatographic method for the determination of propham and chlorpropham in potatoes .
	manualset3
145883	4	409412	5	NULL	NULL	0	NULL	chlorpropham 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple and quick gas chromatographic method for the determination of propham and chlorpropham in potatoes .
	manualset3
145884	5	409412	5	NULL	NULL	0	NULL	potatoes 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple and quick gas chromatographic method for the determination of propham and chlorpropham in potatoes .
	manualset3
145885	1	409413	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data indicate that a less-exposed conformation at A2058 leads to reduction in methylation by ErmE .
	manualset3
145886	2	409413	5	NULL	NULL	0	NULL	less-exposed conformation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data indicate that a less-exposed conformation at A2058 leads to reduction in methylation by ErmE .
	manualset3
145887	3	409413	5	NULL	NULL	0	NULL	A2058 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The data indicate that a less-exposed conformation at A2058 leads to reduction in methylation by ErmE .
	manualset3
145888	4	409413	5	NULL	NULL	NULL	NULL	reduction in methylation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The data indicate that a less-exposed conformation at A2058 leads to reduction in methylation by ErmE .
	manualset3
145889	5	409413	5	NULL	NULL	0	NULL	ErmE	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The data indicate that a less-exposed conformation at A2058 leads to reduction in methylation by ErmE .
	manualset3
145890	1	409414	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data indicate that spx transcription is under negative transcriptional control that is reversed when disulfide stress is encountered .
	manualset3
145891	2	409414	5	NULL	NULL	0	NULL	spx transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data indicate that spx transcription is under negative transcriptional control that is reversed when disulfide stress is encountered .
	manualset3
145892	3	409414	5	NULL	NULL	0	NULL	negative transcriptional control	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data indicate that spx transcription is under negative transcriptional control that is reversed when disulfide stress is encountered .
	manualset3
145893	4	409414	5	NULL	NULL	0	NULL	disulfide stress	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data indicate that spx transcription is under negative transcriptional control that is reversed when disulfide stress is encountered .
	manualset3
145894	1	409415	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data indicated that within the right hemisphere , the magnetoencephalographic ( MEG ) counterpart MMNm of the mismatch negativity ( MMN ) elicited by an infrequent chord change was stronger than the MMNm elicited by a phoneme change .
	manualset3
145895	2	409415	5	NULL	NULL	0	NULL	right hemisphere 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The data indicated that within the right hemisphere , the magnetoencephalographic ( MEG ) counterpart MMNm of the mismatch negativity ( MMN ) elicited by an infrequent chord change was stronger than the MMNm elicited by a phoneme change .
	manualset3
145896	3	409415	5	NULL	NULL	0	NULL	magnetoencephalographic ( MEG ) counterpart MMNm	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data indicated that within the right hemisphere , the magnetoencephalographic ( MEG ) counterpart MMNm of the mismatch negativity ( MMN ) elicited by an infrequent chord change was stronger than the MMNm elicited by a phoneme change .
	manualset3
145897	4	409415	5	NULL	NULL	0	NULL	mismatch negativity ( MMN )	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data indicated that within the right hemisphere , the magnetoencephalographic ( MEG ) counterpart MMNm of the mismatch negativity ( MMN ) elicited by an infrequent chord change was stronger than the MMNm elicited by a phoneme change .
	manualset3
145898	5	409415	5	NULL	NULL	0	NULL	infrequent chord change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data indicated that within the right hemisphere , the magnetoencephalographic ( MEG ) counterpart MMNm of the mismatch negativity ( MMN ) elicited by an infrequent chord change was stronger than the MMNm elicited by a phoneme change .
	manualset3
145899	6	409415	5	NULL	NULL	0	NULL	MMNm 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data indicated that within the right hemisphere , the magnetoencephalographic ( MEG ) counterpart MMNm of the mismatch negativity ( MMN ) elicited by an infrequent chord change was stronger than the MMNm elicited by a phoneme change .
	manualset3
145900	7	409415	5	NULL	NULL	0	NULL	phoneme change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data indicated that within the right hemisphere , the magnetoencephalographic ( MEG ) counterpart MMNm of the mismatch negativity ( MMN ) elicited by an infrequent chord change was stronger than the MMNm elicited by a phoneme change .
	manualset3
145901	1	409416	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained approximated a linear function , as in the previous experiment , but the alignment errors were consistently lower .
	manualset3
145902	2	409416	5	NULL	NULL	0	NULL	linear function	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained approximated a linear function , as in the previous experiment , but the alignment errors were consistently lower .
	manualset3
145903	3	409416	5	NULL	NULL	0	NULL	previous experiment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained approximated a linear function , as in the previous experiment , but the alignment errors were consistently lower .
	manualset3
145904	4	409416	5	NULL	NULL	0	NULL	alignment errors 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained approximated a linear function , as in the previous experiment , but the alignment errors were consistently lower .
	manualset3
145905	1	409417	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained attest to the role of prolonged emotional stress in the genesis of stable metabolic and vasomotor disorders which may promote the development of preconditions for the origin of such cardiovascular diseases as atherosclerosis , hypertensive disease , and coronary thrombosis .
	manualset3
145906	2	409417	5	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained attest to the role of prolonged emotional stress in the genesis of stable metabolic and vasomotor disorders which may promote the development of preconditions for the origin of such cardiovascular diseases as atherosclerosis , hypertensive disease , and coronary thrombosis .
	manualset3
145907	3	409417	5	NULL	NULL	0	NULL	prolonged emotional stress	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained attest to the role of prolonged emotional stress in the genesis of stable metabolic and vasomotor disorders which may promote the development of preconditions for the origin of such cardiovascular diseases as atherosclerosis , hypertensive disease , and coronary thrombosis .
	manualset3
145908	4	409417	5	NULL	NULL	0	NULL	genesis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained attest to the role of prolonged emotional stress in the genesis of stable metabolic and vasomotor disorders which may promote the development of preconditions for the origin of such cardiovascular diseases as atherosclerosis , hypertensive disease , and coronary thrombosis .
	manualset3
145909	5	409417	5	NULL	NULL	0	NULL	stable metabolic disorders 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained attest to the role of prolonged emotional stress in the genesis of stable metabolic and vasomotor disorders which may promote the development of preconditions for the origin of such cardiovascular diseases as atherosclerosis , hypertensive disease , and coronary thrombosis .
	manualset3
145910	6	409417	5	NULL	NULL	0	NULL	vasomotor disorders 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained attest to the role of prolonged emotional stress in the genesis of stable metabolic and vasomotor disorders which may promote the development of preconditions for the origin of such cardiovascular diseases as atherosclerosis , hypertensive disease , and coronary thrombosis .
	manualset3
145911	7	409417	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained attest to the role of prolonged emotional stress in the genesis of stable metabolic and vasomotor disorders which may promote the development of preconditions for the origin of such cardiovascular diseases as atherosclerosis , hypertensive disease , and coronary thrombosis .
	manualset3
145912	8	409417	5	NULL	NULL	0	NULL	preconditions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained attest to the role of prolonged emotional stress in the genesis of stable metabolic and vasomotor disorders which may promote the development of preconditions for the origin of such cardiovascular diseases as atherosclerosis , hypertensive disease , and coronary thrombosis .
	manualset3
145913	9	409417	5	NULL	NULL	0	NULL	origin 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained attest to the role of prolonged emotional stress in the genesis of stable metabolic and vasomotor disorders which may promote the development of preconditions for the origin of such cardiovascular diseases as atherosclerosis , hypertensive disease , and coronary thrombosis .
	manualset3
145914	10	409417	5	NULL	NULL	0	NULL	cardiovascular diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained attest to the role of prolonged emotional stress in the genesis of stable metabolic and vasomotor disorders which may promote the development of preconditions for the origin of such cardiovascular diseases as atherosclerosis , hypertensive disease , and coronary thrombosis .
	manualset3
145915	11	409417	5	NULL	NULL	0	NULL	atherosclerosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained attest to the role of prolonged emotional stress in the genesis of stable metabolic and vasomotor disorders which may promote the development of preconditions for the origin of such cardiovascular diseases as atherosclerosis , hypertensive disease , and coronary thrombosis .
	manualset3
145916	12	409417	5	NULL	NULL	0	NULL	hypertensive disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained attest to the role of prolonged emotional stress in the genesis of stable metabolic and vasomotor disorders which may promote the development of preconditions for the origin of such cardiovascular diseases as atherosclerosis , hypertensive disease , and coronary thrombosis .
	manualset3
145917	13	409417	5	NULL	NULL	0	NULL	coronary thrombosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained attest to the role of prolonged emotional stress in the genesis of stable metabolic and vasomotor disorders which may promote the development of preconditions for the origin of such cardiovascular diseases as atherosclerosis , hypertensive disease , and coronary thrombosis .
	manualset3
145918	1	409418	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained by the psychologist are correlated with the assessment of mental disorders by both the patient himself and the doctor .
	manualset3
145919	2	409418	5	NULL	NULL	0	NULL	psychologist 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained by the psychologist are correlated with the assessment of mental disorders by both the patient himself and the doctor .
	manualset3
145920	3	409418	5	NULL	NULL	0	NULL	assessment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained by the psychologist are correlated with the assessment of mental disorders by both the patient himself and the doctor .
	manualset3
145921	4	409418	5	NULL	NULL	0	NULL	mental disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained by the psychologist are correlated with the assessment of mental disorders by both the patient himself and the doctor .
	manualset3
145922	5	409418	5	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained by the psychologist are correlated with the assessment of mental disorders by both the patient himself and the doctor .
	manualset3
145923	6	409418	5	NULL	NULL	0	NULL	doctor 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained by the psychologist are correlated with the assessment of mental disorders by both the patient himself and the doctor .
	manualset3
145924	1	409419	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained extend the knowledge of the stress-protective functions of low-molecular-weight autoregulators and of the role of intercellular communications in the stress response of bacterial cultures .
	manualset3
145925	2	409419	5	NULL	NULL	0	NULL	knowledge 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained extend the knowledge of the stress-protective functions of low-molecular-weight autoregulators and of the role of intercellular communications in the stress response of bacterial cultures .
	manualset3
145926	3	409419	5	NULL	NULL	0	NULL	stress-protective functions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained extend the knowledge of the stress-protective functions of low-molecular-weight autoregulators and of the role of intercellular communications in the stress response of bacterial cultures .
	manualset3
145927	4	409419	5	NULL	NULL	0	NULL	low-molecular-weight autoregulators	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained extend the knowledge of the stress-protective functions of low-molecular-weight autoregulators and of the role of intercellular communications in the stress response of bacterial cultures .
	manualset3
145928	5	409419	5	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained extend the knowledge of the stress-protective functions of low-molecular-weight autoregulators and of the role of intercellular communications in the stress response of bacterial cultures .
	manualset3
145929	6	409419	5	NULL	NULL	0	NULL	intercellular communications 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained extend the knowledge of the stress-protective functions of low-molecular-weight autoregulators and of the role of intercellular communications in the stress response of bacterial cultures .
	manualset3
145930	7	409419	5	NULL	NULL	0	NULL	stress response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained extend the knowledge of the stress-protective functions of low-molecular-weight autoregulators and of the role of intercellular communications in the stress response of bacterial cultures .
	manualset3
145931	8	409419	5	NULL	NULL	0	NULL	bacterial cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained extend the knowledge of the stress-protective functions of low-molecular-weight autoregulators and of the role of intercellular communications in the stress response of bacterial cultures .
	manualset3
145932	1	409420	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained from this non-randomised study do not support discontinuation and exchange of all drugs used preoperatively in histological poor responders .
	manualset3
145933	2	409420	5	NULL	NULL	0	NULL	non-randomised study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained from this non-randomised study do not support discontinuation and exchange of all drugs used preoperatively in histological poor responders .
	manualset3
145934	3	409420	5	NULL	NULL	0	NULL	discontinuation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained from this non-randomised study do not support discontinuation and exchange of all drugs used preoperatively in histological poor responders .
	manualset3
145935	4	409420	5	NULL	NULL	0	NULL	exchange 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained from this non-randomised study do not support discontinuation and exchange of all drugs used preoperatively in histological poor responders .
	manualset3
145936	5	409420	5	NULL	NULL	0	NULL	drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained from this non-randomised study do not support discontinuation and exchange of all drugs used preoperatively in histological poor responders .
	manualset3
145937	6	409420	5	NULL	NULL	0	NULL	histological poor responders	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained from this non-randomised study do not support discontinuation and exchange of all drugs used preoperatively in histological poor responders .
	manualset3
145938	1	409421	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained showed that beta/gamma-thrombin , deprived of ability to coagulate fibrinogen , maintained its activity towards the other factors of blood coagulation , suggesting the presence of independent hemostatic function in the enzyme .
	manualset3
145939	2	409421	5	NULL	NULL	0	NULL	beta/gamma-thrombin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained showed that beta/gamma-thrombin , deprived of ability to coagulate fibrinogen , maintained its activity towards the other factors of blood coagulation , suggesting the presence of independent hemostatic function in the enzyme .
	manualset3
145940	3	409421	5	NULL	NULL	0	NULL	ability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained showed that beta/gamma-thrombin , deprived of ability to coagulate fibrinogen , maintained its activity towards the other factors of blood coagulation , suggesting the presence of independent hemostatic function in the enzyme .
	manualset3
145941	4	409421	5	NULL	NULL	0	NULL	fibrinogen 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained showed that beta/gamma-thrombin , deprived of ability to coagulate fibrinogen , maintained its activity towards the other factors of blood coagulation , suggesting the presence of independent hemostatic function in the enzyme .
	manualset3
145942	5	409421	5	NULL	NULL	0	NULL	activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained showed that beta/gamma-thrombin , deprived of ability to coagulate fibrinogen , maintained its activity towards the other factors of blood coagulation , suggesting the presence of independent hemostatic function in the enzyme .
	manualset3
145943	6	409421	5	NULL	NULL	0	NULL	factors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained showed that beta/gamma-thrombin , deprived of ability to coagulate fibrinogen , maintained its activity towards the other factors of blood coagulation , suggesting the presence of independent hemostatic function in the enzyme .
	manualset3
145944	7	409421	5	NULL	NULL	0	NULL	blood coagulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained showed that beta/gamma-thrombin , deprived of ability to coagulate fibrinogen , maintained its activity towards the other factors of blood coagulation , suggesting the presence of independent hemostatic function in the enzyme .
	manualset3
145945	8	409421	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained showed that beta/gamma-thrombin , deprived of ability to coagulate fibrinogen , maintained its activity towards the other factors of blood coagulation , suggesting the presence of independent hemostatic function in the enzyme .
	manualset3
145946	9	409421	5	NULL	NULL	0	NULL	independent hemostatic function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained showed that beta/gamma-thrombin , deprived of ability to coagulate fibrinogen , maintained its activity towards the other factors of blood coagulation , suggesting the presence of independent hemostatic function in the enzyme .
	manualset3
145947	10	409421	5	NULL	NULL	0	NULL	enzyme 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The data obtained showed that beta/gamma-thrombin , deprived of ability to coagulate fibrinogen , maintained its activity towards the other factors of blood coagulation , suggesting the presence of independent hemostatic function in the enzyme .
	manualset3
145948	1	409422	5	NULL	NULL	0	NULL	Chronic myocardial ischemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Chronic myocardial ischemia -- hibernating myocardium : characteristics and limits ) .
	manualset3
145949	2	409422	5	NULL	NULL	0	NULL	hibernating myocardium	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	( Chronic myocardial ischemia -- hibernating myocardium : characteristics and limits ) .
	manualset3
145950	3	409422	5	NULL	NULL	0	NULL	characteristics 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Chronic myocardial ischemia -- hibernating myocardium : characteristics and limits ) .
	manualset3
145951	4	409422	5	NULL	NULL	0	NULL	limits 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Chronic myocardial ischemia -- hibernating myocardium : characteristics and limits ) .
	manualset3
145952	1	409423	5	NULL	NULL	0	NULL	method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple and rapid method is described for releasing the epsilon subunit from chloroplast coupling factor 1 by treatment with 20 % ethanol on an anion exchange column .
	manualset3
145953	2	409423	5	NULL	NULL	0	NULL	epsilon subunit 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple and rapid method is described for releasing the epsilon subunit from chloroplast coupling factor 1 by treatment with 20 % ethanol on an anion exchange column .
	manualset3
145954	3	409423	5	NULL	NULL	0	NULL	chloroplast coupling factor 1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple and rapid method is described for releasing the epsilon subunit from chloroplast coupling factor 1 by treatment with 20 % ethanol on an anion exchange column .
	manualset3
145955	4	409423	5	NULL	NULL	0	NULL	treatment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple and rapid method is described for releasing the epsilon subunit from chloroplast coupling factor 1 by treatment with 20 % ethanol on an anion exchange column .
	manualset3
145956	5	409423	5	NULL	NULL	0	NULL	 20 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple and rapid method is described for releasing the epsilon subunit from chloroplast coupling factor 1 by treatment with 20 % ethanol on an anion exchange column .
	manualset3
145957	6	409423	5	NULL	NULL	0	NULL	ethanol 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple and rapid method is described for releasing the epsilon subunit from chloroplast coupling factor 1 by treatment with 20 % ethanol on an anion exchange column .
	manualset3
145958	7	409423	5	NULL	NULL	0	NULL	anion exchange column	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple and rapid method is described for releasing the epsilon subunit from chloroplast coupling factor 1 by treatment with 20 % ethanol on an anion exchange column .
	manualset3
145959	1	409424	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data on L2-E and L3-E interactions are not unequivocal .
	manualset3
145960	2	409424	5	NULL	NULL	0	NULL	L2-E interactions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data on L2-E and L3-E interactions are not unequivocal .
	manualset3
145961	3	409424	5	NULL	NULL	0	NULL	L3-E interactions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data on L2-E and L3-E interactions are not unequivocal .
	manualset3
145962	1	409425	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data provides evidence that the F1-ATPase beta-subunit is the enterostatin receptor and suggests that enterostatin and beta-casomorphin1-7 bind to distinct sites on the protein .
	manualset3
145963	2	409425	5	NULL	NULL	0	NULL	evidence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data provides evidence that the F1-ATPase beta-subunit is the enterostatin receptor and suggests that enterostatin and beta-casomorphin1-7 bind to distinct sites on the protein .
	manualset3
145964	3	409425	5	NULL	NULL	0	NULL	F1-ATPase beta-subunit	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The data provides evidence that the F1-ATPase beta-subunit is the enterostatin receptor and suggests that enterostatin and beta-casomorphin1-7 bind to distinct sites on the protein .
	manualset3
145965	4	409425	5	NULL	NULL	0	NULL	enterostatin receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The data provides evidence that the F1-ATPase beta-subunit is the enterostatin receptor and suggests that enterostatin and beta-casomorphin1-7 bind to distinct sites on the protein .
	manualset3
145966	5	409425	5	NULL	NULL	0	NULL	enterostatin 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The data provides evidence that the F1-ATPase beta-subunit is the enterostatin receptor and suggests that enterostatin and beta-casomorphin1-7 bind to distinct sites on the protein .
	manualset3
145967	6	409425	5	NULL	NULL	0	NULL	beta-casomorphin1-7	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The data provides evidence that the F1-ATPase beta-subunit is the enterostatin receptor and suggests that enterostatin and beta-casomorphin1-7 bind to distinct sites on the protein .
	manualset3
145968	7	409425	5	NULL	NULL	0	NULL	distinct sites 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The data provides evidence that the F1-ATPase beta-subunit is the enterostatin receptor and suggests that enterostatin and beta-casomorphin1-7 bind to distinct sites on the protein .
	manualset3
145969	8	409425	5	NULL	NULL	0	NULL	protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The data provides evidence that the F1-ATPase beta-subunit is the enterostatin receptor and suggests that enterostatin and beta-casomorphin1-7 bind to distinct sites on the protein .
	manualset3
145970	1	409426	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data reveal a previously unrecognized TH-independent major pathway of peripheral dopamine synthesis in young , but not adult , mice .
	manualset3
145971	2	409426	5	NULL	NULL	0	NULL	TH-independent major pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data reveal a previously unrecognized TH-independent major pathway of peripheral dopamine synthesis in young , but not adult , mice .
	manualset3
145972	3	409426	5	NULL	NULL	0	NULL	peripheral dopamine synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data reveal a previously unrecognized TH-independent major pathway of peripheral dopamine synthesis in young , but not adult , mice .
	manualset3
145973	4	409426	5	NULL	NULL	0	NULL	young , but not adult , mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The data reveal a previously unrecognized TH-independent major pathway of peripheral dopamine synthesis in young , but not adult , mice .
	manualset3
145974	1	409427	5	NULL	NULL	0	NULL	data sets 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data sets from 8 laboratories for the 6 key toxins plus DTX1 and DTX2 gave within-laboratories repeatability ( RSD ( R ) ) of 8-12 % , except for PTX-2 .
	manualset3
145975	2	409427	5	NULL	NULL	0	NULL	8 laboratories 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The data sets from 8 laboratories for the 6 key toxins plus DTX1 and DTX2 gave within-laboratories repeatability ( RSD ( R ) ) of 8-12 % , except for PTX-2 .
	manualset3
145976	3	409427	5	NULL	NULL	0	NULL	6 key toxins	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The data sets from 8 laboratories for the 6 key toxins plus DTX1 and DTX2 gave within-laboratories repeatability ( RSD ( R ) ) of 8-12 % , except for PTX-2 .
	manualset3
145977	4	409427	5	NULL	NULL	0	NULL	DTX1 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The data sets from 8 laboratories for the 6 key toxins plus DTX1 and DTX2 gave within-laboratories repeatability ( RSD ( R ) ) of 8-12 % , except for PTX-2 .
	manualset3
145978	5	409427	5	NULL	NULL	0	NULL	DTX2 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The data sets from 8 laboratories for the 6 key toxins plus DTX1 and DTX2 gave within-laboratories repeatability ( RSD ( R ) ) of 8-12 % , except for PTX-2 .
	manualset3
145979	6	409427	5	NULL	NULL	0	NULL	within-laboratories repeatability ( RSD ( R ) )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data sets from 8 laboratories for the 6 key toxins plus DTX1 and DTX2 gave within-laboratories repeatability ( RSD ( R ) ) of 8-12 % , except for PTX-2 .
	manualset3
145980	7	409427	5	NULL	NULL	0	NULL	8-12 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The data sets from 8 laboratories for the 6 key toxins plus DTX1 and DTX2 gave within-laboratories repeatability ( RSD ( R ) ) of 8-12 % , except for PTX-2 .
	manualset3
145981	8	409427	5	NULL	NULL	0	NULL	PTX-2	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The data sets from 8 laboratories for the 6 key toxins plus DTX1 and DTX2 gave within-laboratories repeatability ( RSD ( R ) ) of 8-12 % , except for PTX-2 .
	manualset3
145982	1	409428	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data show that cyclic adenosine monophosphate ( cAMP ) , adenylate cyclase , cAMP phosphodiesterase , and their regulation by intracellular modulators are important to the development of rat lungs .
	manualset3
145983	2	409428	5	NULL	NULL	0	NULL	cyclic adenosine monophosphate ( cAMP ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The data show that cyclic adenosine monophosphate ( cAMP ) , adenylate cyclase , cAMP phosphodiesterase , and their regulation by intracellular modulators are important to the development of rat lungs .
	manualset3
145984	3	409428	5	NULL	NULL	0	NULL	adenylate cyclase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The data show that cyclic adenosine monophosphate ( cAMP ) , adenylate cyclase , cAMP phosphodiesterase , and their regulation by intracellular modulators are important to the development of rat lungs .
	manualset3
145985	4	409428	5	NULL	NULL	0	NULL	cAMP phosphodiesterase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The data show that cyclic adenosine monophosphate ( cAMP ) , adenylate cyclase , cAMP phosphodiesterase , and their regulation by intracellular modulators are important to the development of rat lungs .
	manualset3
145986	5	409428	5	NULL	NULL	0	NULL	regulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data show that cyclic adenosine monophosphate ( cAMP ) , adenylate cyclase , cAMP phosphodiesterase , and their regulation by intracellular modulators are important to the development of rat lungs .
	manualset3
145987	6	409428	5	NULL	NULL	0	NULL	intracellular modulators	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The data show that cyclic adenosine monophosphate ( cAMP ) , adenylate cyclase , cAMP phosphodiesterase , and their regulation by intracellular modulators are important to the development of rat lungs .
	manualset3
145988	7	409428	5	NULL	NULL	0	NULL	development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data show that cyclic adenosine monophosphate ( cAMP ) , adenylate cyclase , cAMP phosphodiesterase , and their regulation by intracellular modulators are important to the development of rat lungs .
	manualset3
145989	8	409428	5	NULL	NULL	0	NULL	rat lungs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The data show that cyclic adenosine monophosphate ( cAMP ) , adenylate cyclase , cAMP phosphodiesterase , and their regulation by intracellular modulators are important to the development of rat lungs .
	manualset3
145990	1	409429	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data showed 87 % of distance was made up of a cyclic activity comprising jogging forwards , then backwards at mean running speeds of 7.2 km x h ( -1 ) and 10.8 km x h ( -1 ) respectively ( made up of 9s bursts on average , each separated by 3s breaks ) .
	manualset3
145991	2	409429	5	NULL	NULL	0	NULL	87 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The data showed 87 % of distance was made up of a cyclic activity comprising jogging forwards , then backwards at mean running speeds of 7.2 km x h ( -1 ) and 10.8 km x h ( -1 ) respectively ( made up of 9s bursts on average , each separated by 3s breaks ) .
	manualset3
145992	3	409429	5	NULL	NULL	0	NULL	distance 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data showed 87 % of distance was made up of a cyclic activity comprising jogging forwards , then backwards at mean running speeds of 7.2 km x h ( -1 ) and 10.8 km x h ( -1 ) respectively ( made up of 9s bursts on average , each separated by 3s breaks ) .
	manualset3
145993	4	409429	5	NULL	NULL	0	NULL	cyclic activity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data showed 87 % of distance was made up of a cyclic activity comprising jogging forwards , then backwards at mean running speeds of 7.2 km x h ( -1 ) and 10.8 km x h ( -1 ) respectively ( made up of 9s bursts on average , each separated by 3s breaks ) .
	manualset3
145994	5	409429	5	NULL	NULL	0	NULL	jogging 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data showed 87 % of distance was made up of a cyclic activity comprising jogging forwards , then backwards at mean running speeds of 7.2 km x h ( -1 ) and 10.8 km x h ( -1 ) respectively ( made up of 9s bursts on average , each separated by 3s breaks ) .
	manualset3
145995	6	409429	5	NULL	NULL	0	NULL	mean running speeds	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data showed 87 % of distance was made up of a cyclic activity comprising jogging forwards , then backwards at mean running speeds of 7.2 km x h ( -1 ) and 10.8 km x h ( -1 ) respectively ( made up of 9s bursts on average , each separated by 3s breaks ) .
	manualset3
145996	7	409429	5	NULL	NULL	0	NULL	7.2 km x h ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The data showed 87 % of distance was made up of a cyclic activity comprising jogging forwards , then backwards at mean running speeds of 7.2 km x h ( -1 ) and 10.8 km x h ( -1 ) respectively ( made up of 9s bursts on average , each separated by 3s breaks ) .
	manualset3
145997	8	409429	5	NULL	NULL	0	NULL	10.8 km x h ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The data showed 87 % of distance was made up of a cyclic activity comprising jogging forwards , then backwards at mean running speeds of 7.2 km x h ( -1 ) and 10.8 km x h ( -1 ) respectively ( made up of 9s bursts on average , each separated by 3s breaks ) .
	manualset3
145998	9	409429	5	NULL	NULL	0	NULL	9s bursts 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The data showed 87 % of distance was made up of a cyclic activity comprising jogging forwards , then backwards at mean running speeds of 7.2 km x h ( -1 ) and 10.8 km x h ( -1 ) respectively ( made up of 9s bursts on average , each separated by 3s breaks ) .
	manualset3
145999	10	409429	5	NULL	NULL	0	NULL	average 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data showed 87 % of distance was made up of a cyclic activity comprising jogging forwards , then backwards at mean running speeds of 7.2 km x h ( -1 ) and 10.8 km x h ( -1 ) respectively ( made up of 9s bursts on average , each separated by 3s breaks ) .
	manualset3
146000	11	409429	5	NULL	NULL	0	NULL	3s breaks 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The data showed 87 % of distance was made up of a cyclic activity comprising jogging forwards , then backwards at mean running speeds of 7.2 km x h ( -1 ) and 10.8 km x h ( -1 ) respectively ( made up of 9s bursts on average , each separated by 3s breaks ) .
	manualset3
146001	1	409430	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data showed that caffeine shortened reaction time .
	manualset3
146002	2	409430	5	NULL	NULL	0	NULL	caffeine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The data showed that caffeine shortened reaction time .
	manualset3
146003	3	409430	5	NULL	NULL	0	NULL	reaction time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The data showed that caffeine shortened reaction time .
	manualset3
146004	1	409431	5	NULL	NULL	0	NULL	restriction patterns	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data showed that the restriction patterns of PstI was most polymorphic among four enzymes ( BamHI , EcoRI , PstI , and SmaI ) used , which revealed 13 types among 25 strains belonged to 4 phage types , 1 untypable and 2 not-determined strains .
	manualset3
146005	2	409431	5	NULL	NULL	0	NULL	PstI 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The data showed that the restriction patterns of PstI was most polymorphic among four enzymes ( BamHI , EcoRI , PstI , and SmaI ) used , which revealed 13 types among 25 strains belonged to 4 phage types , 1 untypable and 2 not-determined strains .
	manualset3
146006	3	409431	5	NULL	NULL	0	NULL	four enzymes	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The data showed that the restriction patterns of PstI was most polymorphic among four enzymes ( BamHI , EcoRI , PstI , and SmaI ) used , which revealed 13 types among 25 strains belonged to 4 phage types , 1 untypable and 2 not-determined strains .
	manualset3
146007	4	409431	5	NULL	NULL	0	NULL	BamHI 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The data showed that the restriction patterns of PstI was most polymorphic among four enzymes ( BamHI , EcoRI , PstI , and SmaI ) used , which revealed 13 types among 25 strains belonged to 4 phage types , 1 untypable and 2 not-determined strains .
	manualset3
146008	5	409431	5	NULL	NULL	0	NULL	EcoRI 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The data showed that the restriction patterns of PstI was most polymorphic among four enzymes ( BamHI , EcoRI , PstI , and SmaI ) used , which revealed 13 types among 25 strains belonged to 4 phage types , 1 untypable and 2 not-determined strains .
	manualset3
146009	6	409431	5	NULL	NULL	0	NULL	PstI 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The data showed that the restriction patterns of PstI was most polymorphic among four enzymes ( BamHI , EcoRI , PstI , and SmaI ) used , which revealed 13 types among 25 strains belonged to 4 phage types , 1 untypable and 2 not-determined strains .
	manualset3
146010	7	409431	5	NULL	NULL	0	NULL	SmaI 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The data showed that the restriction patterns of PstI was most polymorphic among four enzymes ( BamHI , EcoRI , PstI , and SmaI ) used , which revealed 13 types among 25 strains belonged to 4 phage types , 1 untypable and 2 not-determined strains .
	manualset3
146011	8	409431	5	NULL	NULL	0	NULL	13 types 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The data showed that the restriction patterns of PstI was most polymorphic among four enzymes ( BamHI , EcoRI , PstI , and SmaI ) used , which revealed 13 types among 25 strains belonged to 4 phage types , 1 untypable and 2 not-determined strains .
	manualset3
146012	9	409431	5	NULL	NULL	0	NULL	25 strains	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The data showed that the restriction patterns of PstI was most polymorphic among four enzymes ( BamHI , EcoRI , PstI , and SmaI ) used , which revealed 13 types among 25 strains belonged to 4 phage types , 1 untypable and 2 not-determined strains .
	manualset3
146013	10	409431	5	NULL	NULL	0	NULL	 4 phage types	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The data showed that the restriction patterns of PstI was most polymorphic among four enzymes ( BamHI , EcoRI , PstI , and SmaI ) used , which revealed 13 types among 25 strains belonged to 4 phage types , 1 untypable and 2 not-determined strains .
	manualset3
146014	11	409431	5	NULL	NULL	0	NULL	1 untypable	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The data showed that the restriction patterns of PstI was most polymorphic among four enzymes ( BamHI , EcoRI , PstI , and SmaI ) used , which revealed 13 types among 25 strains belonged to 4 phage types , 1 untypable and 2 not-determined strains .
	manualset3
146015	12	409431	5	NULL	NULL	NULL	NULL	2 not-determined strains	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The data showed that the restriction patterns of PstI was most polymorphic among four enzymes ( BamHI , EcoRI , PstI , and SmaI ) used , which revealed 13 types among 25 strains belonged to 4 phage types , 1 untypable and 2 not-determined strains .
	manualset3
146016	1	409432	5	NULL	NULL	0	NULL	method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple and rapid method is described for the determination of AP ( apurinic/apyrimidinic ) sites in DNA .
	manualset3
146017	2	409432	5	NULL	NULL	0	NULL	determination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple and rapid method is described for the determination of AP ( apurinic/apyrimidinic ) sites in DNA .
	manualset3
146018	3	409432	5	NULL	NULL	0	NULL	AP ( apurinic/apyrimidinic ) sites	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple and rapid method is described for the determination of AP ( apurinic/apyrimidinic ) sites in DNA .
	manualset3
146019	4	409432	5	NULL	NULL	0	NULL	DNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple and rapid method is described for the determination of AP ( apurinic/apyrimidinic ) sites in DNA .
	manualset3
146020	1	409433	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that AGEPC produces direct myocardial depression and distinct effects on the coronary and femoral vasculature .
	manualset3
146021	2	409433	5	NULL	NULL	0	NULL	AGEPC 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that AGEPC produces direct myocardial depression and distinct effects on the coronary and femoral vasculature .
	manualset3
146022	3	409433	5	NULL	NULL	0	NULL	direct myocardial depression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that AGEPC produces direct myocardial depression and distinct effects on the coronary and femoral vasculature .
	manualset3
146023	4	409433	5	NULL	NULL	0	NULL	distinct effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that AGEPC produces direct myocardial depression and distinct effects on the coronary and femoral vasculature .
	manualset3
146024	5	409433	5	NULL	NULL	0	NULL	coronary vasculature 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that AGEPC produces direct myocardial depression and distinct effects on the coronary and femoral vasculature .
	manualset3
146025	6	409433	5	NULL	NULL	0	NULL	femoral vasculature 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that AGEPC produces direct myocardial depression and distinct effects on the coronary and femoral vasculature .
	manualset3
146026	1	409434	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that after a few days of cessation of occupational exposure to mercury vapor the HgU before and after administration of DMSA mainly reflects the amount of mercury stored in the kidney , which represents a mercury pool with a slow turnover .
	manualset3
146027	2	409434	5	NULL	NULL	0	NULL	days 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that after a few days of cessation of occupational exposure to mercury vapor the HgU before and after administration of DMSA mainly reflects the amount of mercury stored in the kidney , which represents a mercury pool with a slow turnover .
	manualset3
146028	3	409434	5	NULL	NULL	0	NULL	cessation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that after a few days of cessation of occupational exposure to mercury vapor the HgU before and after administration of DMSA mainly reflects the amount of mercury stored in the kidney , which represents a mercury pool with a slow turnover .
	manualset3
146029	4	409434	5	NULL	NULL	0	NULL	occupational exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that after a few days of cessation of occupational exposure to mercury vapor the HgU before and after administration of DMSA mainly reflects the amount of mercury stored in the kidney , which represents a mercury pool with a slow turnover .
	manualset3
146030	5	409434	5	NULL	NULL	0	NULL	mercury vapor the HgU	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that after a few days of cessation of occupational exposure to mercury vapor the HgU before and after administration of DMSA mainly reflects the amount of mercury stored in the kidney , which represents a mercury pool with a slow turnover .
	manualset3
146031	6	409434	5	NULL	NULL	0	NULL	administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that after a few days of cessation of occupational exposure to mercury vapor the HgU before and after administration of DMSA mainly reflects the amount of mercury stored in the kidney , which represents a mercury pool with a slow turnover .
	manualset3
146032	7	409434	5	NULL	NULL	0	NULL	DMSA 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that after a few days of cessation of occupational exposure to mercury vapor the HgU before and after administration of DMSA mainly reflects the amount of mercury stored in the kidney , which represents a mercury pool with a slow turnover .
	manualset3
146033	8	409434	5	NULL	NULL	0	NULL	amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that after a few days of cessation of occupational exposure to mercury vapor the HgU before and after administration of DMSA mainly reflects the amount of mercury stored in the kidney , which represents a mercury pool with a slow turnover .
	manualset3
146034	9	409434	5	NULL	NULL	0	NULL	mercury 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that after a few days of cessation of occupational exposure to mercury vapor the HgU before and after administration of DMSA mainly reflects the amount of mercury stored in the kidney , which represents a mercury pool with a slow turnover .
	manualset3
146035	10	409434	5	NULL	NULL	0	NULL	kidney 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that after a few days of cessation of occupational exposure to mercury vapor the HgU before and after administration of DMSA mainly reflects the amount of mercury stored in the kidney , which represents a mercury pool with a slow turnover .
	manualset3
146036	11	409434	5	NULL	NULL	0	NULL	mercury pool	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that after a few days of cessation of occupational exposure to mercury vapor the HgU before and after administration of DMSA mainly reflects the amount of mercury stored in the kidney , which represents a mercury pool with a slow turnover .
	manualset3
146037	12	409434	5	NULL	NULL	0	NULL	slow turnover	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that after a few days of cessation of occupational exposure to mercury vapor the HgU before and after administration of DMSA mainly reflects the amount of mercury stored in the kidney , which represents a mercury pool with a slow turnover .
	manualset3
146038	1	409435	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that an important component of ischemia-induced cardiac cell damage in an asanguineous setting is hydrogen peroxide-dependent , and interventions that either inhibit production of superoxide anion or degrade hydrogen peroxide offer best protection .
	manualset3
146039	2	409435	5	NULL	NULL	0	NULL	important component 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that an important component of ischemia-induced cardiac cell damage in an asanguineous setting is hydrogen peroxide-dependent , and interventions that either inhibit production of superoxide anion or degrade hydrogen peroxide offer best protection .
	manualset3
146040	3	409435	5	NULL	NULL	0	NULL	ischemia-induced cardiac cell damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that an important component of ischemia-induced cardiac cell damage in an asanguineous setting is hydrogen peroxide-dependent , and interventions that either inhibit production of superoxide anion or degrade hydrogen peroxide offer best protection .
	manualset3
146041	4	409435	5	NULL	NULL	0	NULL	asanguineous setting	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that an important component of ischemia-induced cardiac cell damage in an asanguineous setting is hydrogen peroxide-dependent , and interventions that either inhibit production of superoxide anion or degrade hydrogen peroxide offer best protection .
	manualset3
146042	5	409435	5	NULL	NULL	0	NULL	interventions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that an important component of ischemia-induced cardiac cell damage in an asanguineous setting is hydrogen peroxide-dependent , and interventions that either inhibit production of superoxide anion or degrade hydrogen peroxide offer best protection .
	manualset3
146043	6	409435	5	NULL	NULL	0	NULL	production 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that an important component of ischemia-induced cardiac cell damage in an asanguineous setting is hydrogen peroxide-dependent , and interventions that either inhibit production of superoxide anion or degrade hydrogen peroxide offer best protection .
	manualset3
146044	7	409435	5	NULL	NULL	0	NULL	superoxide anion	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that an important component of ischemia-induced cardiac cell damage in an asanguineous setting is hydrogen peroxide-dependent , and interventions that either inhibit production of superoxide anion or degrade hydrogen peroxide offer best protection .
	manualset3
146045	8	409435	5	NULL	NULL	0	NULL	hydrogen peroxide	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that an important component of ischemia-induced cardiac cell damage in an asanguineous setting is hydrogen peroxide-dependent , and interventions that either inhibit production of superoxide anion or degrade hydrogen peroxide offer best protection .
	manualset3
146046	9	409435	5	NULL	NULL	0	NULL	protection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that an important component of ischemia-induced cardiac cell damage in an asanguineous setting is hydrogen peroxide-dependent , and interventions that either inhibit production of superoxide anion or degrade hydrogen peroxide offer best protection .
	manualset3
146047	1	409436	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that both PE and NPE possess beta ( 2 ) adrenergic receptors , but only NPE cells possess dopamine D1 receptors linked to Na-K-Cl cotransport .
	manualset3
146048	2	409436	5	NULL	NULL	NULL	NULL	PE 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The data suggest that both PE and NPE possess beta ( 2 ) adrenergic receptors , but only NPE cells possess dopamine D1 receptors linked to Na-K-Cl cotransport .
	manualset3
146049	3	409436	5	NULL	NULL	NULL	NULL	NPE 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The data suggest that both PE and NPE possess beta ( 2 ) adrenergic receptors , but only NPE cells possess dopamine D1 receptors linked to Na-K-Cl cotransport .
	manualset3
146050	4	409436	5	NULL	NULL	NULL	NULL	beta ( 2 ) adrenergic receptors	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The data suggest that both PE and NPE possess beta ( 2 ) adrenergic receptors , but only NPE cells possess dopamine D1 receptors linked to Na-K-Cl cotransport .
	manualset3
146051	5	409436	5	NULL	NULL	0	NULL	NPE cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that both PE and NPE possess beta ( 2 ) adrenergic receptors , but only NPE cells possess dopamine D1 receptors linked to Na-K-Cl cotransport .
	manualset3
146052	6	409436	5	NULL	NULL	0	NULL	dopamine D1 receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that both PE and NPE possess beta ( 2 ) adrenergic receptors , but only NPE cells possess dopamine D1 receptors linked to Na-K-Cl cotransport .
	manualset3
146053	7	409436	5	NULL	NULL	0	NULL	Na-K-Cl cotransport	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that both PE and NPE possess beta ( 2 ) adrenergic receptors , but only NPE cells possess dopamine D1 receptors linked to Na-K-Cl cotransport .
	manualset3
146054	1	409437	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that small RNAs produced during interspecific hybridization or polyploidization serve as a buffer against the genomic shock in interspecific hybrids and allopolyploids : Stable inheritance of repeat-associated siRNAs maintains chromatin and genome stability , whereas expression variation of miRNAs leads to changes in gene expression , growth vigor , and adaptation .
	manualset3
146055	2	409437	5	NULL	NULL	0	NULL	small RNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that small RNAs produced during interspecific hybridization or polyploidization serve as a buffer against the genomic shock in interspecific hybrids and allopolyploids : Stable inheritance of repeat-associated siRNAs maintains chromatin and genome stability , whereas expression variation of miRNAs leads to changes in gene expression , growth vigor , and adaptation .
	manualset3
146056	3	409437	5	NULL	NULL	0	NULL	interspecific hybridization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that small RNAs produced during interspecific hybridization or polyploidization serve as a buffer against the genomic shock in interspecific hybrids and allopolyploids : Stable inheritance of repeat-associated siRNAs maintains chromatin and genome stability , whereas expression variation of miRNAs leads to changes in gene expression , growth vigor , and adaptation .
	manualset3
146057	4	409437	5	NULL	NULL	0	NULL	polyploidization 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that small RNAs produced during interspecific hybridization or polyploidization serve as a buffer against the genomic shock in interspecific hybrids and allopolyploids : Stable inheritance of repeat-associated siRNAs maintains chromatin and genome stability , whereas expression variation of miRNAs leads to changes in gene expression , growth vigor , and adaptation .
	manualset3
146058	5	409437	5	NULL	NULL	0	NULL	buffer 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that small RNAs produced during interspecific hybridization or polyploidization serve as a buffer against the genomic shock in interspecific hybrids and allopolyploids : Stable inheritance of repeat-associated siRNAs maintains chromatin and genome stability , whereas expression variation of miRNAs leads to changes in gene expression , growth vigor , and adaptation .
	manualset3
146059	6	409437	5	NULL	NULL	0	NULL	genomic shock	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that small RNAs produced during interspecific hybridization or polyploidization serve as a buffer against the genomic shock in interspecific hybrids and allopolyploids : Stable inheritance of repeat-associated siRNAs maintains chromatin and genome stability , whereas expression variation of miRNAs leads to changes in gene expression , growth vigor , and adaptation .
	manualset3
146060	7	409437	5	NULL	NULL	NULL	NULL	interspecific hybrids	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The data suggest that small RNAs produced during interspecific hybridization or polyploidization serve as a buffer against the genomic shock in interspecific hybrids and allopolyploids : Stable inheritance of repeat-associated siRNAs maintains chromatin and genome stability , whereas expression variation of miRNAs leads to changes in gene expression , growth vigor , and adaptation .
	manualset3
146061	8	409437	5	NULL	NULL	NULL	NULL	allopolyploids 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The data suggest that small RNAs produced during interspecific hybridization or polyploidization serve as a buffer against the genomic shock in interspecific hybrids and allopolyploids : Stable inheritance of repeat-associated siRNAs maintains chromatin and genome stability , whereas expression variation of miRNAs leads to changes in gene expression , growth vigor , and adaptation .
	manualset3
146062	9	409437	5	NULL	NULL	0	NULL	inheritance 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that small RNAs produced during interspecific hybridization or polyploidization serve as a buffer against the genomic shock in interspecific hybrids and allopolyploids : Stable inheritance of repeat-associated siRNAs maintains chromatin and genome stability , whereas expression variation of miRNAs leads to changes in gene expression , growth vigor , and adaptation .
	manualset3
146063	10	409437	5	NULL	NULL	0	NULL	repeat-associated siRNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that small RNAs produced during interspecific hybridization or polyploidization serve as a buffer against the genomic shock in interspecific hybrids and allopolyploids : Stable inheritance of repeat-associated siRNAs maintains chromatin and genome stability , whereas expression variation of miRNAs leads to changes in gene expression , growth vigor , and adaptation .
	manualset3
146064	11	409437	5	NULL	NULL	0	NULL	chromatin stability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that small RNAs produced during interspecific hybridization or polyploidization serve as a buffer against the genomic shock in interspecific hybrids and allopolyploids : Stable inheritance of repeat-associated siRNAs maintains chromatin and genome stability , whereas expression variation of miRNAs leads to changes in gene expression , growth vigor , and adaptation .
	manualset3
146065	12	409437	5	NULL	NULL	0	NULL	genome stability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that small RNAs produced during interspecific hybridization or polyploidization serve as a buffer against the genomic shock in interspecific hybrids and allopolyploids : Stable inheritance of repeat-associated siRNAs maintains chromatin and genome stability , whereas expression variation of miRNAs leads to changes in gene expression , growth vigor , and adaptation .
	manualset3
146066	13	409437	5	NULL	NULL	0	NULL	expression variation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that small RNAs produced during interspecific hybridization or polyploidization serve as a buffer against the genomic shock in interspecific hybrids and allopolyploids : Stable inheritance of repeat-associated siRNAs maintains chromatin and genome stability , whereas expression variation of miRNAs leads to changes in gene expression , growth vigor , and adaptation .
	manualset3
146067	14	409437	5	NULL	NULL	0	NULL	miRNAs 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that small RNAs produced during interspecific hybridization or polyploidization serve as a buffer against the genomic shock in interspecific hybrids and allopolyploids : Stable inheritance of repeat-associated siRNAs maintains chromatin and genome stability , whereas expression variation of miRNAs leads to changes in gene expression , growth vigor , and adaptation .
	manualset3
146068	15	409437	5	NULL	NULL	0	NULL	changes 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that small RNAs produced during interspecific hybridization or polyploidization serve as a buffer against the genomic shock in interspecific hybrids and allopolyploids : Stable inheritance of repeat-associated siRNAs maintains chromatin and genome stability , whereas expression variation of miRNAs leads to changes in gene expression , growth vigor , and adaptation .
	manualset3
146069	16	409437	5	NULL	NULL	0	NULL	gene expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that small RNAs produced during interspecific hybridization or polyploidization serve as a buffer against the genomic shock in interspecific hybrids and allopolyploids : Stable inheritance of repeat-associated siRNAs maintains chromatin and genome stability , whereas expression variation of miRNAs leads to changes in gene expression , growth vigor , and adaptation .
	manualset3
146070	17	409437	5	NULL	NULL	0	NULL	growth vigor	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that small RNAs produced during interspecific hybridization or polyploidization serve as a buffer against the genomic shock in interspecific hybrids and allopolyploids : Stable inheritance of repeat-associated siRNAs maintains chromatin and genome stability , whereas expression variation of miRNAs leads to changes in gene expression , growth vigor , and adaptation .
	manualset3
146071	18	409437	5	NULL	NULL	0	NULL	adaptation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that small RNAs produced during interspecific hybridization or polyploidization serve as a buffer against the genomic shock in interspecific hybrids and allopolyploids : Stable inheritance of repeat-associated siRNAs maintains chromatin and genome stability , whereas expression variation of miRNAs leads to changes in gene expression , growth vigor , and adaptation .
	manualset3
146072	1	409438	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that the skeletal D3 region is involved in the Ca ( 2 + ) - dependent regulation of the RyR1 channel .
	manualset3
146073	2	409438	5	NULL	NULL	0	NULL	skeletal D3 region 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that the skeletal D3 region is involved in the Ca ( 2 + ) - dependent regulation of the RyR1 channel .
	manualset3
146074	3	409438	5	NULL	NULL	0	NULL	Ca ( 2 + ) - dependent regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that the skeletal D3 region is involved in the Ca ( 2 + ) - dependent regulation of the RyR1 channel .
	manualset3
146075	4	409438	5	NULL	NULL	0	NULL	RyR1 channel 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that the skeletal D3 region is involved in the Ca ( 2 + ) - dependent regulation of the RyR1 channel .
	manualset3
146076	1	409439	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data used in this analysis is from 1061 sites of 8 subjects , with moderate to severe periodontal disease , monitored monthly for about a year .
	manualset3
146077	2	409439	5	NULL	NULL	0	NULL	analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data used in this analysis is from 1061 sites of 8 subjects , with moderate to severe periodontal disease , monitored monthly for about a year .
	manualset3
146078	3	409439	5	NULL	NULL	0	NULL	1061 sites	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The data used in this analysis is from 1061 sites of 8 subjects , with moderate to severe periodontal disease , monitored monthly for about a year .
	manualset3
146079	4	409439	5	NULL	NULL	0	NULL	8 subjects	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The data used in this analysis is from 1061 sites of 8 subjects , with moderate to severe periodontal disease , monitored monthly for about a year .
	manualset3
146080	5	409439	5	NULL	NULL	0	NULL	periodontal disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The data used in this analysis is from 1061 sites of 8 subjects , with moderate to severe periodontal disease , monitored monthly for about a year .
	manualset3
146081	6	409439	5	NULL	NULL	0	NULL	year 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The data used in this analysis is from 1061 sites of 8 subjects , with moderate to severe periodontal disease , monitored monthly for about a year .
	manualset3
146082	1	409440	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data were analyzed with SPM and ICA .
	manualset3
146083	2	409440	5	NULL	NULL	0	NULL	SPM 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data were analyzed with SPM and ICA .
	manualset3
146084	3	409440	5	NULL	NULL	0	NULL	ICA 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data were analyzed with SPM and ICA .
	manualset3
146085	1	409441	5	NULL	NULL	NULL	NULL	simple boundary element computer model	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A simple boundary element computer model suggests that the most even distribution of current flow through the heart is achieved for those electrode locations in which the impedance across the heart is at or near the maximum cardiac impedance for any location of these particular electrodes .
	manualset3
146086	2	409441	5	NULL	NULL	0	NULL	distribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple boundary element computer model suggests that the most even distribution of current flow through the heart is achieved for those electrode locations in which the impedance across the heart is at or near the maximum cardiac impedance for any location of these particular electrodes .
	manualset3
146087	3	409441	5	NULL	NULL	0	NULL	current flow 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple boundary element computer model suggests that the most even distribution of current flow through the heart is achieved for those electrode locations in which the impedance across the heart is at or near the maximum cardiac impedance for any location of these particular electrodes .
	manualset3
146088	4	409441	5	NULL	NULL	0	NULL	heart 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple boundary element computer model suggests that the most even distribution of current flow through the heart is achieved for those electrode locations in which the impedance across the heart is at or near the maximum cardiac impedance for any location of these particular electrodes .
	manualset3
146089	5	409441	5	NULL	NULL	0	NULL	electrode locations	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple boundary element computer model suggests that the most even distribution of current flow through the heart is achieved for those electrode locations in which the impedance across the heart is at or near the maximum cardiac impedance for any location of these particular electrodes .
	manualset3
146090	6	409441	5	NULL	NULL	0	NULL	impedance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple boundary element computer model suggests that the most even distribution of current flow through the heart is achieved for those electrode locations in which the impedance across the heart is at or near the maximum cardiac impedance for any location of these particular electrodes .
	manualset3
146091	7	409441	5	NULL	NULL	0	NULL	heart 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple boundary element computer model suggests that the most even distribution of current flow through the heart is achieved for those electrode locations in which the impedance across the heart is at or near the maximum cardiac impedance for any location of these particular electrodes .
	manualset3
146092	8	409441	5	NULL	NULL	0	NULL	cardiac impedance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple boundary element computer model suggests that the most even distribution of current flow through the heart is achieved for those electrode locations in which the impedance across the heart is at or near the maximum cardiac impedance for any location of these particular electrodes .
	manualset3
146093	9	409441	5	NULL	NULL	0	NULL	location 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple boundary element computer model suggests that the most even distribution of current flow through the heart is achieved for those electrode locations in which the impedance across the heart is at or near the maximum cardiac impedance for any location of these particular electrodes .
	manualset3
146094	10	409441	5	NULL	NULL	0	NULL	particular electrodes 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple boundary element computer model suggests that the most even distribution of current flow through the heart is achieved for those electrode locations in which the impedance across the heart is at or near the maximum cardiac impedance for any location of these particular electrodes .
	manualset3
146095	1	409442	5	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data were obtained on content of calcium and phosphorus in compact part of human tubular bone .
	manualset3
146096	2	409442	5	NULL	NULL	0	NULL	content 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data were obtained on content of calcium and phosphorus in compact part of human tubular bone .
	manualset3
146097	3	409442	5	NULL	NULL	0	NULL	calcium 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The data were obtained on content of calcium and phosphorus in compact part of human tubular bone .
	manualset3
146098	4	409442	5	NULL	NULL	0	NULL	phosphorus 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The data were obtained on content of calcium and phosphorus in compact part of human tubular bone .
	manualset3
146099	5	409442	5	NULL	NULL	0	NULL	compact part of human tubular bone 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The data were obtained on content of calcium and phosphorus in compact part of human tubular bone .
	manualset3
146100	1	409443	5	NULL	NULL	0	NULL	dead patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The dead patients had significantly increased prevalence of cardiac disease ( P less than .02 ) , higher frequency of above-knee amputation ( P less than .01 ) , and a duration of diabetes ( 17.4 + / - 2.8 years ) significantly longer ( P less than .025 ) than that of the surviving patients ( 12.0 + / - 1.0 years ) .
	manualset3
146101	2	409443	5	NULL	NULL	0	NULL	prevalence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dead patients had significantly increased prevalence of cardiac disease ( P less than .02 ) , higher frequency of above-knee amputation ( P less than .01 ) , and a duration of diabetes ( 17.4 + / - 2.8 years ) significantly longer ( P less than .025 ) than that of the surviving patients ( 12.0 + / - 1.0 years ) .
	manualset3
146102	3	409443	5	NULL	NULL	0	NULL	cardiac disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The dead patients had significantly increased prevalence of cardiac disease ( P less than .02 ) , higher frequency of above-knee amputation ( P less than .01 ) , and a duration of diabetes ( 17.4 + / - 2.8 years ) significantly longer ( P less than .025 ) than that of the surviving patients ( 12.0 + / - 1.0 years ) .
	manualset3
146103	4	409443	5	NULL	NULL	0	NULL	 P less than .02 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The dead patients had significantly increased prevalence of cardiac disease ( P less than .02 ) , higher frequency of above-knee amputation ( P less than .01 ) , and a duration of diabetes ( 17.4 + / - 2.8 years ) significantly longer ( P less than .025 ) than that of the surviving patients ( 12.0 + / - 1.0 years ) .
	manualset3
146104	5	409443	5	NULL	NULL	0	NULL	higher frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The dead patients had significantly increased prevalence of cardiac disease ( P less than .02 ) , higher frequency of above-knee amputation ( P less than .01 ) , and a duration of diabetes ( 17.4 + / - 2.8 years ) significantly longer ( P less than .025 ) than that of the surviving patients ( 12.0 + / - 1.0 years ) .
	manualset3
146105	6	409443	5	NULL	NULL	0	NULL	 above-knee amputation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The dead patients had significantly increased prevalence of cardiac disease ( P less than .02 ) , higher frequency of above-knee amputation ( P less than .01 ) , and a duration of diabetes ( 17.4 + / - 2.8 years ) significantly longer ( P less than .025 ) than that of the surviving patients ( 12.0 + / - 1.0 years ) .
	manualset3
146106	7	409443	5	NULL	NULL	0	NULL	P less than .01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The dead patients had significantly increased prevalence of cardiac disease ( P less than .02 ) , higher frequency of above-knee amputation ( P less than .01 ) , and a duration of diabetes ( 17.4 + / - 2.8 years ) significantly longer ( P less than .025 ) than that of the surviving patients ( 12.0 + / - 1.0 years ) .
	manualset3
146107	8	409443	5	NULL	NULL	0	NULL	duration 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The dead patients had significantly increased prevalence of cardiac disease ( P less than .02 ) , higher frequency of above-knee amputation ( P less than .01 ) , and a duration of diabetes ( 17.4 + / - 2.8 years ) significantly longer ( P less than .025 ) than that of the surviving patients ( 12.0 + / - 1.0 years ) .
	manualset3
146108	9	409443	5	NULL	NULL	0	NULL	diabetes 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The dead patients had significantly increased prevalence of cardiac disease ( P less than .02 ) , higher frequency of above-knee amputation ( P less than .01 ) , and a duration of diabetes ( 17.4 + / - 2.8 years ) significantly longer ( P less than .025 ) than that of the surviving patients ( 12.0 + / - 1.0 years ) .
	manualset3
146109	10	409443	5	NULL	NULL	0	NULL	17.4 + / - 2.8 years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The dead patients had significantly increased prevalence of cardiac disease ( P less than .02 ) , higher frequency of above-knee amputation ( P less than .01 ) , and a duration of diabetes ( 17.4 + / - 2.8 years ) significantly longer ( P less than .025 ) than that of the surviving patients ( 12.0 + / - 1.0 years ) .
	manualset3
146110	11	409443	5	NULL	NULL	0	NULL	P less than .025	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The dead patients had significantly increased prevalence of cardiac disease ( P less than .02 ) , higher frequency of above-knee amputation ( P less than .01 ) , and a duration of diabetes ( 17.4 + / - 2.8 years ) significantly longer ( P less than .025 ) than that of the surviving patients ( 12.0 + / - 1.0 years ) .
	manualset3
146111	12	409443	5	NULL	NULL	0	NULL	surviving patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The dead patients had significantly increased prevalence of cardiac disease ( P less than .02 ) , higher frequency of above-knee amputation ( P less than .01 ) , and a duration of diabetes ( 17.4 + / - 2.8 years ) significantly longer ( P less than .025 ) than that of the surviving patients ( 12.0 + / - 1.0 years ) .
	manualset3
146112	13	409443	5	NULL	NULL	0	NULL	12.0 + / - 1.0 years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The dead patients had significantly increased prevalence of cardiac disease ( P less than .02 ) , higher frequency of above-knee amputation ( P less than .01 ) , and a duration of diabetes ( 17.4 + / - 2.8 years ) significantly longer ( P less than .025 ) than that of the surviving patients ( 12.0 + / - 1.0 years ) .
	manualset3
146113	1	409444	5	NULL	NULL	0	NULL	dealkylations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The dealkylations of 7-ethoxy - and 7-pentoxyresorufin , p-nitrophenol hydroxylation , and regio - and stereoselective hydroxylation of testosterone were measured to study the stability and inducibility of cytochrome P450 activities in cultured human hepatocytes .
	manualset3
146114	2	409444	5	NULL	NULL	0	NULL	7-ethoxyresorufin	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The dealkylations of 7-ethoxy - and 7-pentoxyresorufin , p-nitrophenol hydroxylation , and regio - and stereoselective hydroxylation of testosterone were measured to study the stability and inducibility of cytochrome P450 activities in cultured human hepatocytes .
	manualset3
146115	3	409444	5	NULL	NULL	0	NULL	7-pentoxyresorufin	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The dealkylations of 7-ethoxy - and 7-pentoxyresorufin , p-nitrophenol hydroxylation , and regio - and stereoselective hydroxylation of testosterone were measured to study the stability and inducibility of cytochrome P450 activities in cultured human hepatocytes .
	manualset3
146116	4	409444	5	NULL	NULL	0	NULL	p-nitrophenol hydroxylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The dealkylations of 7-ethoxy - and 7-pentoxyresorufin , p-nitrophenol hydroxylation , and regio - and stereoselective hydroxylation of testosterone were measured to study the stability and inducibility of cytochrome P450 activities in cultured human hepatocytes .
	manualset3
146117	5	409444	5	NULL	NULL	0	NULL	regio - and stereoselective hydroxylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The dealkylations of 7-ethoxy - and 7-pentoxyresorufin , p-nitrophenol hydroxylation , and regio - and stereoselective hydroxylation of testosterone were measured to study the stability and inducibility of cytochrome P450 activities in cultured human hepatocytes .
	manualset3
146118	6	409444	5	NULL	NULL	0	NULL	testosterone 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The dealkylations of 7-ethoxy - and 7-pentoxyresorufin , p-nitrophenol hydroxylation , and regio - and stereoselective hydroxylation of testosterone were measured to study the stability and inducibility of cytochrome P450 activities in cultured human hepatocytes .
	manualset3
146119	7	409444	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The dealkylations of 7-ethoxy - and 7-pentoxyresorufin , p-nitrophenol hydroxylation , and regio - and stereoselective hydroxylation of testosterone were measured to study the stability and inducibility of cytochrome P450 activities in cultured human hepatocytes .
	manualset3
146120	8	409444	5	NULL	NULL	0	NULL	stability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dealkylations of 7-ethoxy - and 7-pentoxyresorufin , p-nitrophenol hydroxylation , and regio - and stereoselective hydroxylation of testosterone were measured to study the stability and inducibility of cytochrome P450 activities in cultured human hepatocytes .
	manualset3
146121	9	409444	5	NULL	NULL	0	NULL	inducibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dealkylations of 7-ethoxy - and 7-pentoxyresorufin , p-nitrophenol hydroxylation , and regio - and stereoselective hydroxylation of testosterone were measured to study the stability and inducibility of cytochrome P450 activities in cultured human hepatocytes .
	manualset3
146122	10	409444	5	NULL	NULL	0	NULL	cytochrome P450 activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The dealkylations of 7-ethoxy - and 7-pentoxyresorufin , p-nitrophenol hydroxylation , and regio - and stereoselective hydroxylation of testosterone were measured to study the stability and inducibility of cytochrome P450 activities in cultured human hepatocytes .
	manualset3
146123	11	409444	5	NULL	NULL	0	NULL	cultured human hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The dealkylations of 7-ethoxy - and 7-pentoxyresorufin , p-nitrophenol hydroxylation , and regio - and stereoselective hydroxylation of testosterone were measured to study the stability and inducibility of cytochrome P450 activities in cultured human hepatocytes .
	manualset3
146124	1	409445	5	NULL	NULL	0	NULL	death 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The death in such cases has been attributed to a combination of a high CO2 and a low O2 tension .
	manualset3
146125	2	409445	5	NULL	NULL	0	NULL	cases 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The death in such cases has been attributed to a combination of a high CO2 and a low O2 tension .
	manualset3
146126	3	409445	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The death in such cases has been attributed to a combination of a high CO2 and a low O2 tension .
	manualset3
146127	4	409445	5	NULL	NULL	0	NULL	high CO2 tension 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The death in such cases has been attributed to a combination of a high CO2 and a low O2 tension .
	manualset3
146128	5	409445	5	NULL	NULL	0	NULL	low O2 tension 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The death in such cases has been attributed to a combination of a high CO2 and a low O2 tension .
	manualset3
146129	1	409446	5	NULL	NULL	0	NULL	death ligand TRAIL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The death ligand TRAIL in diabetic nephropathy .
	manualset3
146130	2	409446	5	NULL	NULL	0	NULL	diabetic nephropathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The death ligand TRAIL in diabetic nephropathy .
	manualset3
146131	1	409447	5	NULL	NULL	0	NULL	decisive factor	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The decisive factor in the appearance of postinfection abscesses is the presence of damaged tissues , open to the penetration of microorganisms not only by the exogenic or endogenic route , but also by the so-called exoendogenic route , when they penetrate the body from the air via the upper respiratory ways and further into the blood and damaged tissues .
	manualset3
146132	2	409447	5	NULL	NULL	0	NULL	appearance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The decisive factor in the appearance of postinfection abscesses is the presence of damaged tissues , open to the penetration of microorganisms not only by the exogenic or endogenic route , but also by the so-called exoendogenic route , when they penetrate the body from the air via the upper respiratory ways and further into the blood and damaged tissues .
	manualset3
146133	3	409447	5	NULL	NULL	0	NULL	postinfection abscesses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The decisive factor in the appearance of postinfection abscesses is the presence of damaged tissues , open to the penetration of microorganisms not only by the exogenic or endogenic route , but also by the so-called exoendogenic route , when they penetrate the body from the air via the upper respiratory ways and further into the blood and damaged tissues .
	manualset3
146134	4	409447	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The decisive factor in the appearance of postinfection abscesses is the presence of damaged tissues , open to the penetration of microorganisms not only by the exogenic or endogenic route , but also by the so-called exoendogenic route , when they penetrate the body from the air via the upper respiratory ways and further into the blood and damaged tissues .
	manualset3
146135	5	409447	5	NULL	NULL	0	NULL	damaged tissues 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The decisive factor in the appearance of postinfection abscesses is the presence of damaged tissues , open to the penetration of microorganisms not only by the exogenic or endogenic route , but also by the so-called exoendogenic route , when they penetrate the body from the air via the upper respiratory ways and further into the blood and damaged tissues .
	manualset3
146136	6	409447	5	NULL	NULL	0	NULL	penetration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The decisive factor in the appearance of postinfection abscesses is the presence of damaged tissues , open to the penetration of microorganisms not only by the exogenic or endogenic route , but also by the so-called exoendogenic route , when they penetrate the body from the air via the upper respiratory ways and further into the blood and damaged tissues .
	manualset3
146137	7	409447	5	NULL	NULL	0	NULL	microorganisms 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The decisive factor in the appearance of postinfection abscesses is the presence of damaged tissues , open to the penetration of microorganisms not only by the exogenic or endogenic route , but also by the so-called exoendogenic route , when they penetrate the body from the air via the upper respiratory ways and further into the blood and damaged tissues .
	manualset3
146138	8	409447	5	NULL	NULL	0	NULL	exogenic route 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The decisive factor in the appearance of postinfection abscesses is the presence of damaged tissues , open to the penetration of microorganisms not only by the exogenic or endogenic route , but also by the so-called exoendogenic route , when they penetrate the body from the air via the upper respiratory ways and further into the blood and damaged tissues .
	manualset3
146139	9	409447	5	NULL	NULL	0	NULL	endogenic route 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The decisive factor in the appearance of postinfection abscesses is the presence of damaged tissues , open to the penetration of microorganisms not only by the exogenic or endogenic route , but also by the so-called exoendogenic route , when they penetrate the body from the air via the upper respiratory ways and further into the blood and damaged tissues .
	manualset3
146140	10	409447	5	NULL	NULL	0	NULL	exoendogenic route	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The decisive factor in the appearance of postinfection abscesses is the presence of damaged tissues , open to the penetration of microorganisms not only by the exogenic or endogenic route , but also by the so-called exoendogenic route , when they penetrate the body from the air via the upper respiratory ways and further into the blood and damaged tissues .
	manualset3
146141	11	409447	5	NULL	NULL	0	NULL	body 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The decisive factor in the appearance of postinfection abscesses is the presence of damaged tissues , open to the penetration of microorganisms not only by the exogenic or endogenic route , but also by the so-called exoendogenic route , when they penetrate the body from the air via the upper respiratory ways and further into the blood and damaged tissues .
	manualset3
146142	12	409447	5	NULL	NULL	0	NULL	air 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The decisive factor in the appearance of postinfection abscesses is the presence of damaged tissues , open to the penetration of microorganisms not only by the exogenic or endogenic route , but also by the so-called exoendogenic route , when they penetrate the body from the air via the upper respiratory ways and further into the blood and damaged tissues .
	manualset3
146143	13	409447	5	NULL	NULL	0	NULL	upper respiratory ways 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The decisive factor in the appearance of postinfection abscesses is the presence of damaged tissues , open to the penetration of microorganisms not only by the exogenic or endogenic route , but also by the so-called exoendogenic route , when they penetrate the body from the air via the upper respiratory ways and further into the blood and damaged tissues .
	manualset3
146144	14	409447	5	NULL	NULL	0	NULL	blood 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The decisive factor in the appearance of postinfection abscesses is the presence of damaged tissues , open to the penetration of microorganisms not only by the exogenic or endogenic route , but also by the so-called exoendogenic route , when they penetrate the body from the air via the upper respiratory ways and further into the blood and damaged tissues .
	manualset3
146145	15	409447	5	NULL	NULL	0	NULL	damaged tissues 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The decisive factor in the appearance of postinfection abscesses is the presence of damaged tissues , open to the penetration of microorganisms not only by the exogenic or endogenic route , but also by the so-called exoendogenic route , when they penetrate the body from the air via the upper respiratory ways and further into the blood and damaged tissues .
	manualset3
146146	1	409448	5	NULL	NULL	0	NULL	decomposition 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The decomposition and oxidation of methanol on the macroporous catalyst surfaces with different Pt and Ru molar ratios ( Pt100Ru0 , Pt90Ru10 , Pt80Ru20 , Pt70Ru30 and Pt56Ru44 ) were systemically discussed .
	manualset3
146147	2	409448	5	NULL	NULL	0	NULL	oxidation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The decomposition and oxidation of methanol on the macroporous catalyst surfaces with different Pt and Ru molar ratios ( Pt100Ru0 , Pt90Ru10 , Pt80Ru20 , Pt70Ru30 and Pt56Ru44 ) were systemically discussed .
	manualset3
146148	3	409448	5	NULL	NULL	0	NULL	methanol 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The decomposition and oxidation of methanol on the macroporous catalyst surfaces with different Pt and Ru molar ratios ( Pt100Ru0 , Pt90Ru10 , Pt80Ru20 , Pt70Ru30 and Pt56Ru44 ) were systemically discussed .
	manualset3
146149	4	409448	5	NULL	NULL	0	NULL	macroporous catalyst surfaces 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The decomposition and oxidation of methanol on the macroporous catalyst surfaces with different Pt and Ru molar ratios ( Pt100Ru0 , Pt90Ru10 , Pt80Ru20 , Pt70Ru30 and Pt56Ru44 ) were systemically discussed .
	manualset3
146150	5	409448	5	NULL	NULL	0	NULL	Pt and Ru molar ratios	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The decomposition and oxidation of methanol on the macroporous catalyst surfaces with different Pt and Ru molar ratios ( Pt100Ru0 , Pt90Ru10 , Pt80Ru20 , Pt70Ru30 and Pt56Ru44 ) were systemically discussed .
	manualset3
146151	6	409448	5	NULL	NULL	0	NULL	Pt100Ru0 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The decomposition and oxidation of methanol on the macroporous catalyst surfaces with different Pt and Ru molar ratios ( Pt100Ru0 , Pt90Ru10 , Pt80Ru20 , Pt70Ru30 and Pt56Ru44 ) were systemically discussed .
	manualset3
146152	7	409448	5	NULL	NULL	0	NULL	Pt90Ru10 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The decomposition and oxidation of methanol on the macroporous catalyst surfaces with different Pt and Ru molar ratios ( Pt100Ru0 , Pt90Ru10 , Pt80Ru20 , Pt70Ru30 and Pt56Ru44 ) were systemically discussed .
	manualset3
146153	8	409448	5	NULL	NULL	0	NULL	Pt80Ru20 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The decomposition and oxidation of methanol on the macroporous catalyst surfaces with different Pt and Ru molar ratios ( Pt100Ru0 , Pt90Ru10 , Pt80Ru20 , Pt70Ru30 and Pt56Ru44 ) were systemically discussed .
	manualset3
146154	9	409448	5	NULL	NULL	0	NULL	Pt70Ru30 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The decomposition and oxidation of methanol on the macroporous catalyst surfaces with different Pt and Ru molar ratios ( Pt100Ru0 , Pt90Ru10 , Pt80Ru20 , Pt70Ru30 and Pt56Ru44 ) were systemically discussed .
	manualset3
146155	10	409448	5	NULL	NULL	0	NULL	Pt56Ru44 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The decomposition and oxidation of methanol on the macroporous catalyst surfaces with different Pt and Ru molar ratios ( Pt100Ru0 , Pt90Ru10 , Pt80Ru20 , Pt70Ru30 and Pt56Ru44 ) were systemically discussed .
	manualset3
146157	2	409449	5	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease in binding following purification was restored by histone 2B .
	manualset3
146158	3	409449	5	NULL	NULL	0	NULL	purification 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease in binding following purification was restored by histone 2B .
	manualset3
146159	4	409449	5	NULL	NULL	0	NULL	histone 2B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease in binding following purification was restored by histone 2B .
	manualset3
148669	5	409449	5	NULL	NULL	0	NULL	decrease 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease in binding following purification was restored by histone 2B .
	manualset3
146161	2	409450	5	NULL	NULL	0	NULL	fluorescence 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease in fluorescence reflects the change in environment of the unique tryptophan residue , Trp 311 , during the dimer to monomer dissociation .
	manualset3
146162	3	409450	5	NULL	NULL	0	NULL	change 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease in fluorescence reflects the change in environment of the unique tryptophan residue , Trp 311 , during the dimer to monomer dissociation .
	manualset3
146163	4	409450	5	NULL	NULL	0	NULL	environment 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease in fluorescence reflects the change in environment of the unique tryptophan residue , Trp 311 , during the dimer to monomer dissociation .
	manualset3
146164	5	409450	5	NULL	NULL	0	NULL	unique tryptophan residue , Trp 311	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease in fluorescence reflects the change in environment of the unique tryptophan residue , Trp 311 , during the dimer to monomer dissociation .
	manualset3
146165	6	409450	5	NULL	NULL	0	NULL	dimer to monomer dissociation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease in fluorescence reflects the change in environment of the unique tryptophan residue , Trp 311 , during the dimer to monomer dissociation .
	manualset3
146167	2	409451	5	NULL	NULL	0	NULL	membrane potential	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease in membrane potential by ouabain , up to 20 mV maximum , occurred within 2-5 sec and was not accompanied by detectable changes in input resistance .
	manualset3
146168	3	409451	5	NULL	NULL	0	NULL	ouabain 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease in membrane potential by ouabain , up to 20 mV maximum , occurred within 2-5 sec and was not accompanied by detectable changes in input resistance .
	manualset3
146169	4	409451	5	NULL	NULL	0	NULL	20 mV 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease in membrane potential by ouabain , up to 20 mV maximum , occurred within 2-5 sec and was not accompanied by detectable changes in input resistance .
	manualset3
146170	5	409451	5	NULL	NULL	0	NULL	2-5 sec	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease in membrane potential by ouabain , up to 20 mV maximum , occurred within 2-5 sec and was not accompanied by detectable changes in input resistance .
	manualset3
146171	6	409451	5	NULL	NULL	0	NULL	detectable changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease in membrane potential by ouabain , up to 20 mV maximum , occurred within 2-5 sec and was not accompanied by detectable changes in input resistance .
	manualset3
146172	7	409451	5	NULL	NULL	0	NULL	input resistance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease in membrane potential by ouabain , up to 20 mV maximum , occurred within 2-5 sec and was not accompanied by detectable changes in input resistance .
	manualset3
146174	1	409452	5	NULL	NULL	NULL	NULL	intestinal P-gp expression levels	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The decrease in the intestinal P-gp expression levels were suppressed by aminoguanidine , a specific iNOS inhibitor .
	manualset3
146175	2	409452	5	NULL	NULL	NULL	NULL	aminoguanidine , a specific iNOS inhibitor	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The decrease in the intestinal P-gp expression levels were suppressed by aminoguanidine , a specific iNOS inhibitor .
	manualset3
146177	2	409453	5	NULL	NULL	0	NULL	rate of fibronectin production 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease in the rate of fibronectin and collagen production ( main proteins of intercellular substance ) in fibroblasts with the chromosomes anomalies might be responsible for irreversible impairments of the embryo development , resulting in spontaneous abortion .
	manualset3
146178	3	409453	5	NULL	NULL	0	NULL	rate of collagen production	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease in the rate of fibronectin and collagen production ( main proteins of intercellular substance ) in fibroblasts with the chromosomes anomalies might be responsible for irreversible impairments of the embryo development , resulting in spontaneous abortion .
	manualset3
146179	4	409453	5	NULL	NULL	0	NULL	proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease in the rate of fibronectin and collagen production ( main proteins of intercellular substance ) in fibroblasts with the chromosomes anomalies might be responsible for irreversible impairments of the embryo development , resulting in spontaneous abortion .
	manualset3
146180	5	409453	5	NULL	NULL	0	NULL	intercellular substance	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease in the rate of fibronectin and collagen production ( main proteins of intercellular substance ) in fibroblasts with the chromosomes anomalies might be responsible for irreversible impairments of the embryo development , resulting in spontaneous abortion .
	manualset3
146181	6	409453	5	NULL	NULL	0	NULL	fibroblasts 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease in the rate of fibronectin and collagen production ( main proteins of intercellular substance ) in fibroblasts with the chromosomes anomalies might be responsible for irreversible impairments of the embryo development , resulting in spontaneous abortion .
	manualset3
146182	7	409453	5	NULL	NULL	0	NULL	chromosomes anomalies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease in the rate of fibronectin and collagen production ( main proteins of intercellular substance ) in fibroblasts with the chromosomes anomalies might be responsible for irreversible impairments of the embryo development , resulting in spontaneous abortion .
	manualset3
146183	8	409453	5	NULL	NULL	0	NULL	irreversible impairments	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease in the rate of fibronectin and collagen production ( main proteins of intercellular substance ) in fibroblasts with the chromosomes anomalies might be responsible for irreversible impairments of the embryo development , resulting in spontaneous abortion .
	manualset3
146184	9	409453	5	NULL	NULL	0	NULL	embryo development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease in the rate of fibronectin and collagen production ( main proteins of intercellular substance ) in fibroblasts with the chromosomes anomalies might be responsible for irreversible impairments of the embryo development , resulting in spontaneous abortion .
	manualset3
146185	10	409453	5	NULL	NULL	0	NULL	spontaneous abortion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease in the rate of fibronectin and collagen production ( main proteins of intercellular substance ) in fibroblasts with the chromosomes anomalies might be responsible for irreversible impairments of the embryo development , resulting in spontaneous abortion .
	manualset3
146187	2	409454	5	NULL	NULL	0	NULL	CO2 - radical quantity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease of CO2 - radical quantity in bones of experimental animals have shown , that due to simulation of microgravity the decrease of `` collagen-nanocrystals '' interaction takes place .
	manualset3
146188	3	409454	5	NULL	NULL	0	NULL	bones 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease of CO2 - radical quantity in bones of experimental animals have shown , that due to simulation of microgravity the decrease of `` collagen-nanocrystals '' interaction takes place .
	manualset3
146189	4	409454	5	NULL	NULL	0	NULL	experimental animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease of CO2 - radical quantity in bones of experimental animals have shown , that due to simulation of microgravity the decrease of `` collagen-nanocrystals '' interaction takes place .
	manualset3
146190	5	409454	5	NULL	NULL	0	NULL	simulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease of CO2 - radical quantity in bones of experimental animals have shown , that due to simulation of microgravity the decrease of `` collagen-nanocrystals '' interaction takes place .
	manualset3
146191	6	409454	5	NULL	NULL	0	NULL	microgravity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease of CO2 - radical quantity in bones of experimental animals have shown , that due to simulation of microgravity the decrease of `` collagen-nanocrystals '' interaction takes place .
	manualset3
146192	7	409454	5	NULL	NULL	0	NULL	decrease 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease of CO2 - radical quantity in bones of experimental animals have shown , that due to simulation of microgravity the decrease of `` collagen-nanocrystals '' interaction takes place .
	manualset3
146193	8	409454	5	NULL	NULL	0	NULL	`` collagen-nanocrystals '' interaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease of CO2 - radical quantity in bones of experimental animals have shown , that due to simulation of microgravity the decrease of `` collagen-nanocrystals '' interaction takes place .
	manualset3
146194	1	409455	5	NULL	NULL	0	NULL	resting MP	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease of resting MP after denervation in diaphragm muscle of the rat was studied in vitro .
	manualset3
146195	2	409455	5	NULL	NULL	0	NULL	denervation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease of resting MP after denervation in diaphragm muscle of the rat was studied in vitro .
	manualset3
146196	3	409455	5	NULL	NULL	0	NULL	diaphragm muscle	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease of resting MP after denervation in diaphragm muscle of the rat was studied in vitro .
	manualset3
146197	4	409455	5	NULL	NULL	0	NULL	rat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease of resting MP after denervation in diaphragm muscle of the rat was studied in vitro .
	manualset3
148670	5	409455	5	NULL	NULL	0	NULL	decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The decrease of resting MP after denervation in diaphragm muscle of the rat was studied in vitro .
	manualset3
146198	1	409456	5	NULL	NULL	0	NULL	decreased dye response	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The decreased dye response is not due to the proximity of the crosslinked proteins since the monomers generated after bisection of the crosslinkers with beta-mercaptoethanol show reduced staining .
	manualset3
146199	2	409456	5	NULL	NULL	0	NULL	proximity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The decreased dye response is not due to the proximity of the crosslinked proteins since the monomers generated after bisection of the crosslinkers with beta-mercaptoethanol show reduced staining .
	manualset3
146200	3	409456	5	NULL	NULL	0	NULL	crosslinked proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The decreased dye response is not due to the proximity of the crosslinked proteins since the monomers generated after bisection of the crosslinkers with beta-mercaptoethanol show reduced staining .
	manualset3
146201	4	409456	5	NULL	NULL	0	NULL	monomers 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The decreased dye response is not due to the proximity of the crosslinked proteins since the monomers generated after bisection of the crosslinkers with beta-mercaptoethanol show reduced staining .
	manualset3
146202	5	409456	5	NULL	NULL	0	NULL	bisection 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The decreased dye response is not due to the proximity of the crosslinked proteins since the monomers generated after bisection of the crosslinkers with beta-mercaptoethanol show reduced staining .
	manualset3
146203	6	409456	5	NULL	NULL	0	NULL	crosslinkers 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The decreased dye response is not due to the proximity of the crosslinked proteins since the monomers generated after bisection of the crosslinkers with beta-mercaptoethanol show reduced staining .
	manualset3
146204	7	409456	5	NULL	NULL	0	NULL	beta-mercaptoethanol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The decreased dye response is not due to the proximity of the crosslinked proteins since the monomers generated after bisection of the crosslinkers with beta-mercaptoethanol show reduced staining .
	manualset3
146205	8	409456	5	NULL	NULL	0	NULL	staining 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The decreased dye response is not due to the proximity of the crosslinked proteins since the monomers generated after bisection of the crosslinkers with beta-mercaptoethanol show reduced staining .
	manualset3
146206	1	409457	5	NULL	NULL	0	NULL	whether 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The decreases were identical whether determined by iodine binding or enzyme assay .
	manualset3
146207	2	409457	5	NULL	NULL	0	NULL	iodine binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The decreases were identical whether determined by iodine binding or enzyme assay .
	manualset3
146208	3	409457	5	NULL	NULL	0	NULL	enzyme assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The decreases were identical whether determined by iodine binding or enzyme assay .
	manualset3
148671	4	409457	5	NULL	NULL	0	NULL	decreases	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The decreases were identical whether determined by iodine binding or enzyme assay .
	manualset3
146209	1	409458	5	NULL	NULL	NULL	NULL	amino acid sequence	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The deduced amino acid sequence indicated that aprI codes for a precursor of 715 amino acids and the precursor is composed of four regions including a signal peptide , an N-terminal pro-region , a mature protease region and a C-terminal extension region of 215 amino acids as previously described for aprII ( H. Tsujibo et al. , Gene , 136 , 247-251 ( 1993 ) ) .
	manualset3
146210	2	409458	5	NULL	NULL	0	NULL	aprI 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The deduced amino acid sequence indicated that aprI codes for a precursor of 715 amino acids and the precursor is composed of four regions including a signal peptide , an N-terminal pro-region , a mature protease region and a C-terminal extension region of 215 amino acids as previously described for aprII ( H. Tsujibo et al. , Gene , 136 , 247-251 ( 1993 ) ) .
	manualset3
146211	3	409458	5	NULL	NULL	0	NULL	precursor of 715 amino acids	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The deduced amino acid sequence indicated that aprI codes for a precursor of 715 amino acids and the precursor is composed of four regions including a signal peptide , an N-terminal pro-region , a mature protease region and a C-terminal extension region of 215 amino acids as previously described for aprII ( H. Tsujibo et al. , Gene , 136 , 247-251 ( 1993 ) ) .
	manualset3
146212	4	409458	5	NULL	NULL	0	NULL	precursor 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The deduced amino acid sequence indicated that aprI codes for a precursor of 715 amino acids and the precursor is composed of four regions including a signal peptide , an N-terminal pro-region , a mature protease region and a C-terminal extension region of 215 amino acids as previously described for aprII ( H. Tsujibo et al. , Gene , 136 , 247-251 ( 1993 ) ) .
	manualset3
146213	5	409458	5	NULL	NULL	0	NULL	four regions 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The deduced amino acid sequence indicated that aprI codes for a precursor of 715 amino acids and the precursor is composed of four regions including a signal peptide , an N-terminal pro-region , a mature protease region and a C-terminal extension region of 215 amino acids as previously described for aprII ( H. Tsujibo et al. , Gene , 136 , 247-251 ( 1993 ) ) .
	manualset3
146214	6	409458	5	NULL	NULL	0	NULL	signal peptide	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The deduced amino acid sequence indicated that aprI codes for a precursor of 715 amino acids and the precursor is composed of four regions including a signal peptide , an N-terminal pro-region , a mature protease region and a C-terminal extension region of 215 amino acids as previously described for aprII ( H. Tsujibo et al. , Gene , 136 , 247-251 ( 1993 ) ) .
	manualset3
146215	7	409458	5	NULL	NULL	0	NULL	N-terminal pro-region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The deduced amino acid sequence indicated that aprI codes for a precursor of 715 amino acids and the precursor is composed of four regions including a signal peptide , an N-terminal pro-region , a mature protease region and a C-terminal extension region of 215 amino acids as previously described for aprII ( H. Tsujibo et al. , Gene , 136 , 247-251 ( 1993 ) ) .
	manualset3
146216	8	409458	5	NULL	NULL	0	NULL	mature protease region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The deduced amino acid sequence indicated that aprI codes for a precursor of 715 amino acids and the precursor is composed of four regions including a signal peptide , an N-terminal pro-region , a mature protease region and a C-terminal extension region of 215 amino acids as previously described for aprII ( H. Tsujibo et al. , Gene , 136 , 247-251 ( 1993 ) ) .
	manualset3
146217	9	409458	5	NULL	NULL	0	NULL	C-terminal extension region of 215 amino acids 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The deduced amino acid sequence indicated that aprI codes for a precursor of 715 amino acids and the precursor is composed of four regions including a signal peptide , an N-terminal pro-region , a mature protease region and a C-terminal extension region of 215 amino acids as previously described for aprII ( H. Tsujibo et al. , Gene , 136 , 247-251 ( 1993 ) ) .
	manualset3
146218	10	409458	5	NULL	NULL	0	NULL	aprII 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The deduced amino acid sequence indicated that aprI codes for a precursor of 715 amino acids and the precursor is composed of four regions including a signal peptide , an N-terminal pro-region , a mature protease region and a C-terminal extension region of 215 amino acids as previously described for aprII ( H. Tsujibo et al. , Gene , 136 , 247-251 ( 1993 ) ) .
	manualset3
146219	11	409458	5	NULL	NULL	0	NULL	H. Tsujibo et al. , Gene , 136 , 247-251 ( 1993 ) 	Citation												NULL		0	NULL	NULL	NULL	NULL	NULL	The deduced amino acid sequence indicated that aprI codes for a precursor of 715 amino acids and the precursor is composed of four regions including a signal peptide , an N-terminal pro-region , a mature protease region and a C-terminal extension region of 215 amino acids as previously described for aprII ( H. Tsujibo et al. , Gene , 136 , 247-251 ( 1993 ) ) .
	manualset3
146220	1	409459	5	NULL	NULL	0	NULL	deduced amino acid sequence	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The deduced amino acid sequence of Atlantic cod ATF3 shares over 45 % identity with its putative orthologs from other vertebrates .
	manualset3
146221	2	409459	5	NULL	NULL	0	NULL	Atlantic cod ATF3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The deduced amino acid sequence of Atlantic cod ATF3 shares over 45 % identity with its putative orthologs from other vertebrates .
	manualset3
146222	3	409459	5	NULL	NULL	0	NULL	45 % identity	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The deduced amino acid sequence of Atlantic cod ATF3 shares over 45 % identity with its putative orthologs from other vertebrates .
	manualset3
146223	4	409459	5	NULL	NULL	0	NULL	putative orthologs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The deduced amino acid sequence of Atlantic cod ATF3 shares over 45 % identity with its putative orthologs from other vertebrates .
	manualset3
146224	5	409459	5	NULL	NULL	0	NULL	vertebrates 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The deduced amino acid sequence of Atlantic cod ATF3 shares over 45 % identity with its putative orthologs from other vertebrates .
	manualset3
146225	1	409460	5	NULL	NULL	0	NULL	deficit syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The deficit syndrome and eye tracking disorder may reflect a distinct subtype within the syndrome of schizophrenia .
	manualset3
146226	2	409460	5	NULL	NULL	0	NULL	eye tracking disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The deficit syndrome and eye tracking disorder may reflect a distinct subtype within the syndrome of schizophrenia .
	manualset3
146227	3	409460	5	NULL	NULL	0	NULL	distinct subtype	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The deficit syndrome and eye tracking disorder may reflect a distinct subtype within the syndrome of schizophrenia .
	manualset3
146228	4	409460	5	NULL	NULL	0	NULL	syndrome of schizophrenia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The deficit syndrome and eye tracking disorder may reflect a distinct subtype within the syndrome of schizophrenia .
	manualset3
146229	1	409461	5	NULL	NULL	0	NULL	definition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The definition of weight maintenance .
	manualset3
146230	2	409461	5	NULL	NULL	0	NULL	weight maintenance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The definition of weight maintenance .
	manualset3
146231	1	409462	5	NULL	NULL	0	NULL	degradation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The degradation ( as assessed by measuring UV absorbance ) , the generation of hydroxyl radicals ( as assessed measuring H ( 2 ) O ( 2 ) concentration ) , the mineralization ( in terms of TOC and COD removal ) , and the aerobic biodegradability ( as assessed by the BOD ( 5 ) / COD ratio ) were monitored during sonication .
	manualset3
146232	2	409462	5	NULL	NULL	0	NULL	UV absorbance	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The degradation ( as assessed by measuring UV absorbance ) , the generation of hydroxyl radicals ( as assessed measuring H ( 2 ) O ( 2 ) concentration ) , the mineralization ( in terms of TOC and COD removal ) , and the aerobic biodegradability ( as assessed by the BOD ( 5 ) / COD ratio ) were monitored during sonication .
	manualset3
146233	3	409462	5	NULL	NULL	0	NULL	generation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The degradation ( as assessed by measuring UV absorbance ) , the generation of hydroxyl radicals ( as assessed measuring H ( 2 ) O ( 2 ) concentration ) , the mineralization ( in terms of TOC and COD removal ) , and the aerobic biodegradability ( as assessed by the BOD ( 5 ) / COD ratio ) were monitored during sonication .
	manualset3
146234	4	409462	5	NULL	NULL	0	NULL	hydroxyl radicals 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The degradation ( as assessed by measuring UV absorbance ) , the generation of hydroxyl radicals ( as assessed measuring H ( 2 ) O ( 2 ) concentration ) , the mineralization ( in terms of TOC and COD removal ) , and the aerobic biodegradability ( as assessed by the BOD ( 5 ) / COD ratio ) were monitored during sonication .
	manualset3
146235	5	409462	5	NULL	NULL	0	NULL	H ( 2 ) O ( 2 ) concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The degradation ( as assessed by measuring UV absorbance ) , the generation of hydroxyl radicals ( as assessed measuring H ( 2 ) O ( 2 ) concentration ) , the mineralization ( in terms of TOC and COD removal ) , and the aerobic biodegradability ( as assessed by the BOD ( 5 ) / COD ratio ) were monitored during sonication .
	manualset3
146236	6	409462	5	NULL	NULL	0	NULL	mineralization 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The degradation ( as assessed by measuring UV absorbance ) , the generation of hydroxyl radicals ( as assessed measuring H ( 2 ) O ( 2 ) concentration ) , the mineralization ( in terms of TOC and COD removal ) , and the aerobic biodegradability ( as assessed by the BOD ( 5 ) / COD ratio ) were monitored during sonication .
	manualset3
146237	7	409462	5	NULL	NULL	0	NULL	TOC 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The degradation ( as assessed by measuring UV absorbance ) , the generation of hydroxyl radicals ( as assessed measuring H ( 2 ) O ( 2 ) concentration ) , the mineralization ( in terms of TOC and COD removal ) , and the aerobic biodegradability ( as assessed by the BOD ( 5 ) / COD ratio ) were monitored during sonication .
	manualset3
146238	8	409462	5	NULL	NULL	0	NULL	COD removal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The degradation ( as assessed by measuring UV absorbance ) , the generation of hydroxyl radicals ( as assessed measuring H ( 2 ) O ( 2 ) concentration ) , the mineralization ( in terms of TOC and COD removal ) , and the aerobic biodegradability ( as assessed by the BOD ( 5 ) / COD ratio ) were monitored during sonication .
	manualset3
146239	9	409462	5	NULL	NULL	0	NULL	aerobic biodegradability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The degradation ( as assessed by measuring UV absorbance ) , the generation of hydroxyl radicals ( as assessed measuring H ( 2 ) O ( 2 ) concentration ) , the mineralization ( in terms of TOC and COD removal ) , and the aerobic biodegradability ( as assessed by the BOD ( 5 ) / COD ratio ) were monitored during sonication .
	manualset3
146240	10	409462	5	NULL	NULL	0	NULL	BOD ( 5 ) / COD ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The degradation ( as assessed by measuring UV absorbance ) , the generation of hydroxyl radicals ( as assessed measuring H ( 2 ) O ( 2 ) concentration ) , the mineralization ( in terms of TOC and COD removal ) , and the aerobic biodegradability ( as assessed by the BOD ( 5 ) / COD ratio ) were monitored during sonication .
	manualset3
146241	11	409462	5	NULL	NULL	0	NULL	sonication 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The degradation ( as assessed by measuring UV absorbance ) , the generation of hydroxyl radicals ( as assessed measuring H ( 2 ) O ( 2 ) concentration ) , the mineralization ( in terms of TOC and COD removal ) , and the aerobic biodegradability ( as assessed by the BOD ( 5 ) / COD ratio ) were monitored during sonication .
	manualset3
146242	1	409463	5	NULL	NULL	0	NULL	degradation process	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The degradation process is temperature - and Ca2 + - dependent and has a pH optimum of 6.5-7 .0 .
	manualset3
146243	2	409463	5	NULL	NULL	0	NULL	temperature 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The degradation process is temperature - and Ca2 + - dependent and has a pH optimum of 6.5-7 .0 .
	manualset3
146244	3	409463	5	NULL	NULL	0	NULL	Ca2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The degradation process is temperature - and Ca2 + - dependent and has a pH optimum of 6.5-7 .0 .
	manualset3
146245	4	409463	5	NULL	NULL	0	NULL	pH optimum	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The degradation process is temperature - and Ca2 + - dependent and has a pH optimum of 6.5-7 .0 .
	manualset3
146246	5	409463	5	NULL	NULL	0	NULL	6.5-7 .0	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The degradation process is temperature - and Ca2 + - dependent and has a pH optimum of 6.5-7 .0 .
	manualset3
146247	1	409464	5	NULL	NULL	0	NULL	degrading cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The degrading cells , which by design were identical to the sensing cells , were located in distinct microcolonies on the root surface or in intercellular crevices between the root epidermal cells .
	manualset3
146248	2	409464	5	NULL	NULL	0	NULL	sensing cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The degrading cells , which by design were identical to the sensing cells , were located in distinct microcolonies on the root surface or in intercellular crevices between the root epidermal cells .
	manualset3
146249	3	409464	5	NULL	NULL	0	NULL	distinct microcolonies 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The degrading cells , which by design were identical to the sensing cells , were located in distinct microcolonies on the root surface or in intercellular crevices between the root epidermal cells .
	manualset3
146250	4	409464	5	NULL	NULL	0	NULL	root surface	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The degrading cells , which by design were identical to the sensing cells , were located in distinct microcolonies on the root surface or in intercellular crevices between the root epidermal cells .
	manualset3
146251	5	409464	5	NULL	NULL	0	NULL	intercellular crevices	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The degrading cells , which by design were identical to the sensing cells , were located in distinct microcolonies on the root surface or in intercellular crevices between the root epidermal cells .
	manualset3
146252	6	409464	5	NULL	NULL	0	NULL	root epidermal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The degrading cells , which by design were identical to the sensing cells , were located in distinct microcolonies on the root surface or in intercellular crevices between the root epidermal cells .
	manualset3
146253	1	409465	5	NULL	NULL	0	NULL	degree 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of TCR down-regulation mediated by APL-MHC interactions correlates well with the induction of specific T cell effector functions .
	manualset3
146254	2	409465	5	NULL	NULL	0	NULL	TCR down-regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of TCR down-regulation mediated by APL-MHC interactions correlates well with the induction of specific T cell effector functions .
	manualset3
146255	3	409465	5	NULL	NULL	0	NULL	APL-MHC interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of TCR down-regulation mediated by APL-MHC interactions correlates well with the induction of specific T cell effector functions .
	manualset3
146256	4	409465	5	NULL	NULL	0	NULL	induction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of TCR down-regulation mediated by APL-MHC interactions correlates well with the induction of specific T cell effector functions .
	manualset3
146257	5	409465	5	NULL	NULL	0	NULL	specific T cell effector functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of TCR down-regulation mediated by APL-MHC interactions correlates well with the induction of specific T cell effector functions .
	manualset3
146258	1	409466	5	NULL	NULL	0	NULL	degree 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of binding was dependent on serum albumin levels , ligand concentrations and non-esterified fatty acids ( NEFA ) .
	manualset3
146259	2	409466	5	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of binding was dependent on serum albumin levels , ligand concentrations and non-esterified fatty acids ( NEFA ) .
	manualset3
146260	3	409466	5	NULL	NULL	0	NULL	serum albumin levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of binding was dependent on serum albumin levels , ligand concentrations and non-esterified fatty acids ( NEFA ) .
	manualset3
146261	4	409466	5	NULL	NULL	0	NULL	ligand concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of binding was dependent on serum albumin levels , ligand concentrations and non-esterified fatty acids ( NEFA ) .
	manualset3
146262	5	409466	5	NULL	NULL	0	NULL	non-esterified fatty acids ( NEFA )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of binding was dependent on serum albumin levels , ligand concentrations and non-esterified fatty acids ( NEFA ) .
	manualset3
146263	1	409467	5	NULL	NULL	0	NULL	degree 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of cross-reactivity did not change significantly when the SS , CT , and FPIA assays were calibrated with CsG instead of CsA -- whether parent CsG was present or not .
	manualset3
146264	2	409467	5	NULL	NULL	0	NULL	cross-reactivity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of cross-reactivity did not change significantly when the SS , CT , and FPIA assays were calibrated with CsG instead of CsA -- whether parent CsG was present or not .
	manualset3
146265	3	409467	5	NULL	NULL	0	NULL	SS assays 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of cross-reactivity did not change significantly when the SS , CT , and FPIA assays were calibrated with CsG instead of CsA -- whether parent CsG was present or not .
	manualset3
146266	4	409467	5	NULL	NULL	0	NULL	CT assays 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of cross-reactivity did not change significantly when the SS , CT , and FPIA assays were calibrated with CsG instead of CsA -- whether parent CsG was present or not .
	manualset3
146267	5	409467	5	NULL	NULL	0	NULL	FPIA assays 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of cross-reactivity did not change significantly when the SS , CT , and FPIA assays were calibrated with CsG instead of CsA -- whether parent CsG was present or not .
	manualset3
146268	6	409467	5	NULL	NULL	0	NULL	CsG 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of cross-reactivity did not change significantly when the SS , CT , and FPIA assays were calibrated with CsG instead of CsA -- whether parent CsG was present or not .
	manualset3
146269	7	409467	5	NULL	NULL	0	NULL	CsA 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of cross-reactivity did not change significantly when the SS , CT , and FPIA assays were calibrated with CsG instead of CsA -- whether parent CsG was present or not .
	manualset3
146270	8	409467	5	NULL	NULL	0	NULL	parent CsG	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of cross-reactivity did not change significantly when the SS , CT , and FPIA assays were calibrated with CsG instead of CsA -- whether parent CsG was present or not .
	manualset3
146271	1	409468	5	NULL	NULL	0	NULL	degree of inhibition	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of inhibition was considerably less than that produced by PGI2 , which elevates cAMP .
	manualset3
146272	2	409468	5	NULL	NULL	0	NULL	PGI2 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of inhibition was considerably less than that produced by PGI2 , which elevates cAMP .
	manualset3
146273	3	409468	5	NULL	NULL	0	NULL	cAMP 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of inhibition was considerably less than that produced by PGI2 , which elevates cAMP .
	manualset3
146274	1	409469	5	NULL	NULL	0	NULL	degree of protonation 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of protonation strongly affects the structure , distribution , and the dynamic behavior of confined water and electrolytes .
	manualset3
146275	2	409469	5	NULL	NULL	0	NULL	structure 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of protonation strongly affects the structure , distribution , and the dynamic behavior of confined water and electrolytes .
	manualset3
146276	3	409469	5	NULL	NULL	0	NULL	distribution 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of protonation strongly affects the structure , distribution , and the dynamic behavior of confined water and electrolytes .
	manualset3
146277	4	409469	5	NULL	NULL	0	NULL	dynamic behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of protonation strongly affects the structure , distribution , and the dynamic behavior of confined water and electrolytes .
	manualset3
146278	5	409469	5	NULL	NULL	0	NULL	confined water 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of protonation strongly affects the structure , distribution , and the dynamic behavior of confined water and electrolytes .
	manualset3
146279	6	409469	5	NULL	NULL	0	NULL	electrolytes 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of protonation strongly affects the structure , distribution , and the dynamic behavior of confined water and electrolytes .
	manualset3
146280	1	409470	5	NULL	NULL	0	NULL	degree 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree to which immature cortical networks attempt to compensate for altered levels of physiological activity , as documented in the present report , is another indication of how important such activity can be for normal development ( see Corner , M.A. , van Pelt , J. , Wolters , P.S. , Baker , R.E. and Nuytinck , R.H. ( 2002 ) Physiological e. ects of sustained blockade of excitatory synaptic transmission on spontaneously active developing neuronal networks-an inquiry into the reciprocal linkage between intrinsic biorhythms and neuroplasticity in early ontogeny .
	manualset3
146281	2	409470	5	NULL	NULL	0	NULL	immature cortical networks	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree to which immature cortical networks attempt to compensate for altered levels of physiological activity , as documented in the present report , is another indication of how important such activity can be for normal development ( see Corner , M.A. , van Pelt , J. , Wolters , P.S. , Baker , R.E. and Nuytinck , R.H. ( 2002 ) Physiological e. ects of sustained blockade of excitatory synaptic transmission on spontaneously active developing neuronal networks-an inquiry into the reciprocal linkage between intrinsic biorhythms and neuroplasticity in early ontogeny .
	manualset3
146282	3	409470	5	NULL	NULL	0	NULL	altered levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree to which immature cortical networks attempt to compensate for altered levels of physiological activity , as documented in the present report , is another indication of how important such activity can be for normal development ( see Corner , M.A. , van Pelt , J. , Wolters , P.S. , Baker , R.E. and Nuytinck , R.H. ( 2002 ) Physiological e. ects of sustained blockade of excitatory synaptic transmission on spontaneously active developing neuronal networks-an inquiry into the reciprocal linkage between intrinsic biorhythms and neuroplasticity in early ontogeny .
	manualset3
146283	4	409470	5	NULL	NULL	0	NULL	physiological activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree to which immature cortical networks attempt to compensate for altered levels of physiological activity , as documented in the present report , is another indication of how important such activity can be for normal development ( see Corner , M.A. , van Pelt , J. , Wolters , P.S. , Baker , R.E. and Nuytinck , R.H. ( 2002 ) Physiological e. ects of sustained blockade of excitatory synaptic transmission on spontaneously active developing neuronal networks-an inquiry into the reciprocal linkage between intrinsic biorhythms and neuroplasticity in early ontogeny .
	manualset3
146284	5	409470	5	NULL	NULL	0	NULL	present report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree to which immature cortical networks attempt to compensate for altered levels of physiological activity , as documented in the present report , is another indication of how important such activity can be for normal development ( see Corner , M.A. , van Pelt , J. , Wolters , P.S. , Baker , R.E. and Nuytinck , R.H. ( 2002 ) Physiological e. ects of sustained blockade of excitatory synaptic transmission on spontaneously active developing neuronal networks-an inquiry into the reciprocal linkage between intrinsic biorhythms and neuroplasticity in early ontogeny .
	manualset3
146285	6	409470	5	NULL	NULL	0	NULL	indication 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree to which immature cortical networks attempt to compensate for altered levels of physiological activity , as documented in the present report , is another indication of how important such activity can be for normal development ( see Corner , M.A. , van Pelt , J. , Wolters , P.S. , Baker , R.E. and Nuytinck , R.H. ( 2002 ) Physiological e. ects of sustained blockade of excitatory synaptic transmission on spontaneously active developing neuronal networks-an inquiry into the reciprocal linkage between intrinsic biorhythms and neuroplasticity in early ontogeny .
	manualset3
146286	7	409470	5	NULL	NULL	0	NULL	activity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree to which immature cortical networks attempt to compensate for altered levels of physiological activity , as documented in the present report , is another indication of how important such activity can be for normal development ( see Corner , M.A. , van Pelt , J. , Wolters , P.S. , Baker , R.E. and Nuytinck , R.H. ( 2002 ) Physiological e. ects of sustained blockade of excitatory synaptic transmission on spontaneously active developing neuronal networks-an inquiry into the reciprocal linkage between intrinsic biorhythms and neuroplasticity in early ontogeny .
	manualset3
146287	8	409470	5	NULL	NULL	0	NULL	normal development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree to which immature cortical networks attempt to compensate for altered levels of physiological activity , as documented in the present report , is another indication of how important such activity can be for normal development ( see Corner , M.A. , van Pelt , J. , Wolters , P.S. , Baker , R.E. and Nuytinck , R.H. ( 2002 ) Physiological e. ects of sustained blockade of excitatory synaptic transmission on spontaneously active developing neuronal networks-an inquiry into the reciprocal linkage between intrinsic biorhythms and neuroplasticity in early ontogeny .
	manualset3
146288	9	409470	5	NULL	NULL	0	NULL	Corner , M.A. , van Pelt , J. , Wolters , P.S. , Baker , R.E. and Nuytinck , R.H. ( 2002 ) 	Citation												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree to which immature cortical networks attempt to compensate for altered levels of physiological activity , as documented in the present report , is another indication of how important such activity can be for normal development ( see Corner , M.A. , van Pelt , J. , Wolters , P.S. , Baker , R.E. and Nuytinck , R.H. ( 2002 ) Physiological e. ects of sustained blockade of excitatory synaptic transmission on spontaneously active developing neuronal networks-an inquiry into the reciprocal linkage between intrinsic biorhythms and neuroplasticity in early ontogeny .
	manualset3
146289	10	409470	5	NULL	NULL	0	NULL	Physiological e. ects 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree to which immature cortical networks attempt to compensate for altered levels of physiological activity , as documented in the present report , is another indication of how important such activity can be for normal development ( see Corner , M.A. , van Pelt , J. , Wolters , P.S. , Baker , R.E. and Nuytinck , R.H. ( 2002 ) Physiological e. ects of sustained blockade of excitatory synaptic transmission on spontaneously active developing neuronal networks-an inquiry into the reciprocal linkage between intrinsic biorhythms and neuroplasticity in early ontogeny .
	manualset3
146290	11	409470	5	NULL	NULL	0	NULL	blockade 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree to which immature cortical networks attempt to compensate for altered levels of physiological activity , as documented in the present report , is another indication of how important such activity can be for normal development ( see Corner , M.A. , van Pelt , J. , Wolters , P.S. , Baker , R.E. and Nuytinck , R.H. ( 2002 ) Physiological e. ects of sustained blockade of excitatory synaptic transmission on spontaneously active developing neuronal networks-an inquiry into the reciprocal linkage between intrinsic biorhythms and neuroplasticity in early ontogeny .
	manualset3
146291	12	409470	5	NULL	NULL	0	NULL	excitatory synaptic transmission	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree to which immature cortical networks attempt to compensate for altered levels of physiological activity , as documented in the present report , is another indication of how important such activity can be for normal development ( see Corner , M.A. , van Pelt , J. , Wolters , P.S. , Baker , R.E. and Nuytinck , R.H. ( 2002 ) Physiological e. ects of sustained blockade of excitatory synaptic transmission on spontaneously active developing neuronal networks-an inquiry into the reciprocal linkage between intrinsic biorhythms and neuroplasticity in early ontogeny .
	manualset3
146292	13	409470	5	NULL	NULL	NULL	NULL	neuronal networks	AnatomicalPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The degree to which immature cortical networks attempt to compensate for altered levels of physiological activity , as documented in the present report , is another indication of how important such activity can be for normal development ( see Corner , M.A. , van Pelt , J. , Wolters , P.S. , Baker , R.E. and Nuytinck , R.H. ( 2002 ) Physiological e. ects of sustained blockade of excitatory synaptic transmission on spontaneously active developing neuronal networks-an inquiry into the reciprocal linkage between intrinsic biorhythms and neuroplasticity in early ontogeny .
	manualset3
146293	14	409470	5	NULL	NULL	0	NULL	inquiry 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree to which immature cortical networks attempt to compensate for altered levels of physiological activity , as documented in the present report , is another indication of how important such activity can be for normal development ( see Corner , M.A. , van Pelt , J. , Wolters , P.S. , Baker , R.E. and Nuytinck , R.H. ( 2002 ) Physiological e. ects of sustained blockade of excitatory synaptic transmission on spontaneously active developing neuronal networks-an inquiry into the reciprocal linkage between intrinsic biorhythms and neuroplasticity in early ontogeny .
	manualset3
146294	15	409470	5	NULL	NULL	0	NULL	reciprocal linkage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree to which immature cortical networks attempt to compensate for altered levels of physiological activity , as documented in the present report , is another indication of how important such activity can be for normal development ( see Corner , M.A. , van Pelt , J. , Wolters , P.S. , Baker , R.E. and Nuytinck , R.H. ( 2002 ) Physiological e. ects of sustained blockade of excitatory synaptic transmission on spontaneously active developing neuronal networks-an inquiry into the reciprocal linkage between intrinsic biorhythms and neuroplasticity in early ontogeny .
	manualset3
146295	16	409470	5	NULL	NULL	0	NULL	intrinsic biorhythms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree to which immature cortical networks attempt to compensate for altered levels of physiological activity , as documented in the present report , is another indication of how important such activity can be for normal development ( see Corner , M.A. , van Pelt , J. , Wolters , P.S. , Baker , R.E. and Nuytinck , R.H. ( 2002 ) Physiological e. ects of sustained blockade of excitatory synaptic transmission on spontaneously active developing neuronal networks-an inquiry into the reciprocal linkage between intrinsic biorhythms and neuroplasticity in early ontogeny .
	manualset3
146296	17	409470	5	NULL	NULL	0	NULL	neuroplasticity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree to which immature cortical networks attempt to compensate for altered levels of physiological activity , as documented in the present report , is another indication of how important such activity can be for normal development ( see Corner , M.A. , van Pelt , J. , Wolters , P.S. , Baker , R.E. and Nuytinck , R.H. ( 2002 ) Physiological e. ects of sustained blockade of excitatory synaptic transmission on spontaneously active developing neuronal networks-an inquiry into the reciprocal linkage between intrinsic biorhythms and neuroplasticity in early ontogeny .
	manualset3
146297	18	409470	5	NULL	NULL	0	NULL	 early ontogeny 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree to which immature cortical networks attempt to compensate for altered levels of physiological activity , as documented in the present report , is another indication of how important such activity can be for normal development ( see Corner , M.A. , van Pelt , J. , Wolters , P.S. , Baker , R.E. and Nuytinck , R.H. ( 2002 ) Physiological e. ects of sustained blockade of excitatory synaptic transmission on spontaneously active developing neuronal networks-an inquiry into the reciprocal linkage between intrinsic biorhythms and neuroplasticity in early ontogeny .
	manualset3
146298	1	409471	5	NULL	NULL	0	NULL	dehydrating effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dehydrating effect of DMSO explains the results of a previous study , confirmed in this study , that increasing the concentration of DMSO raises the main transition temperature and eliminates the ripple phase .
	manualset3
146299	2	409471	5	NULL	NULL	0	NULL	DMSO 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The dehydrating effect of DMSO explains the results of a previous study , confirmed in this study , that increasing the concentration of DMSO raises the main transition temperature and eliminates the ripple phase .
	manualset3
146300	3	409471	5	NULL	NULL	0	NULL	results 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The dehydrating effect of DMSO explains the results of a previous study , confirmed in this study , that increasing the concentration of DMSO raises the main transition temperature and eliminates the ripple phase .
	manualset3
146301	4	409471	5	NULL	NULL	0	NULL	previous study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The dehydrating effect of DMSO explains the results of a previous study , confirmed in this study , that increasing the concentration of DMSO raises the main transition temperature and eliminates the ripple phase .
	manualset3
146302	5	409471	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The dehydrating effect of DMSO explains the results of a previous study , confirmed in this study , that increasing the concentration of DMSO raises the main transition temperature and eliminates the ripple phase .
	manualset3
146303	6	409471	5	NULL	NULL	0	NULL	concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The dehydrating effect of DMSO explains the results of a previous study , confirmed in this study , that increasing the concentration of DMSO raises the main transition temperature and eliminates the ripple phase .
	manualset3
146304	7	409471	5	NULL	NULL	0	NULL	DMSO 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The dehydrating effect of DMSO explains the results of a previous study , confirmed in this study , that increasing the concentration of DMSO raises the main transition temperature and eliminates the ripple phase .
	manualset3
146305	8	409471	5	NULL	NULL	0	NULL	transition temperature 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The dehydrating effect of DMSO explains the results of a previous study , confirmed in this study , that increasing the concentration of DMSO raises the main transition temperature and eliminates the ripple phase .
	manualset3
146306	9	409471	5	NULL	NULL	0	NULL	ripple phase 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The dehydrating effect of DMSO explains the results of a previous study , confirmed in this study , that increasing the concentration of DMSO raises the main transition temperature and eliminates the ripple phase .
	manualset3
146307	1	409472	5	NULL	NULL	0	NULL	delay for admission	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The delay for admission was comparable for the two groups .
	manualset3
146308	2	409472	5	NULL	NULL	0	NULL	two groups	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The delay for admission was comparable for the two groups .
	manualset3
146309	1	409473	5	NULL	NULL	0	NULL	delay 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The delay observed between admission to hospital and first symptoms , together with the presence of anatomical lesions or physiological disturbances suggesting bacterial invasion by the intestinal route , have led the authors to postulate a nosocomial digestive contamination , probably from water , as suggested by the particular ecology of this micro-organism .
	manualset3
146310	2	409473	5	NULL	NULL	0	NULL	admission 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The delay observed between admission to hospital and first symptoms , together with the presence of anatomical lesions or physiological disturbances suggesting bacterial invasion by the intestinal route , have led the authors to postulate a nosocomial digestive contamination , probably from water , as suggested by the particular ecology of this micro-organism .
	manualset3
146311	3	409473	5	NULL	NULL	0	NULL	hospital 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The delay observed between admission to hospital and first symptoms , together with the presence of anatomical lesions or physiological disturbances suggesting bacterial invasion by the intestinal route , have led the authors to postulate a nosocomial digestive contamination , probably from water , as suggested by the particular ecology of this micro-organism .
	manualset3
146312	4	409473	5	NULL	NULL	0	NULL	symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The delay observed between admission to hospital and first symptoms , together with the presence of anatomical lesions or physiological disturbances suggesting bacterial invasion by the intestinal route , have led the authors to postulate a nosocomial digestive contamination , probably from water , as suggested by the particular ecology of this micro-organism .
	manualset3
146313	5	409473	5	NULL	NULL	0	NULL	anatomical lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The delay observed between admission to hospital and first symptoms , together with the presence of anatomical lesions or physiological disturbances suggesting bacterial invasion by the intestinal route , have led the authors to postulate a nosocomial digestive contamination , probably from water , as suggested by the particular ecology of this micro-organism .
	manualset3
146314	6	409473	5	NULL	NULL	0	NULL	physiological disturbances	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The delay observed between admission to hospital and first symptoms , together with the presence of anatomical lesions or physiological disturbances suggesting bacterial invasion by the intestinal route , have led the authors to postulate a nosocomial digestive contamination , probably from water , as suggested by the particular ecology of this micro-organism .
	manualset3
146315	7	409473	5	NULL	NULL	0	NULL	bacterial invasion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The delay observed between admission to hospital and first symptoms , together with the presence of anatomical lesions or physiological disturbances suggesting bacterial invasion by the intestinal route , have led the authors to postulate a nosocomial digestive contamination , probably from water , as suggested by the particular ecology of this micro-organism .
	manualset3
146316	8	409473	5	NULL	NULL	0	NULL	intestinal route	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The delay observed between admission to hospital and first symptoms , together with the presence of anatomical lesions or physiological disturbances suggesting bacterial invasion by the intestinal route , have led the authors to postulate a nosocomial digestive contamination , probably from water , as suggested by the particular ecology of this micro-organism .
	manualset3
146317	9	409473	5	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The delay observed between admission to hospital and first symptoms , together with the presence of anatomical lesions or physiological disturbances suggesting bacterial invasion by the intestinal route , have led the authors to postulate a nosocomial digestive contamination , probably from water , as suggested by the particular ecology of this micro-organism .
	manualset3
146318	10	409473	5	NULL	NULL	0	NULL	nosocomial digestive contamination	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The delay observed between admission to hospital and first symptoms , together with the presence of anatomical lesions or physiological disturbances suggesting bacterial invasion by the intestinal route , have led the authors to postulate a nosocomial digestive contamination , probably from water , as suggested by the particular ecology of this micro-organism .
	manualset3
146319	11	409473	5	NULL	NULL	0	NULL	water 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The delay observed between admission to hospital and first symptoms , together with the presence of anatomical lesions or physiological disturbances suggesting bacterial invasion by the intestinal route , have led the authors to postulate a nosocomial digestive contamination , probably from water , as suggested by the particular ecology of this micro-organism .
	manualset3
146320	12	409473	5	NULL	NULL	0	NULL	particular ecology	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The delay observed between admission to hospital and first symptoms , together with the presence of anatomical lesions or physiological disturbances suggesting bacterial invasion by the intestinal route , have led the authors to postulate a nosocomial digestive contamination , probably from water , as suggested by the particular ecology of this micro-organism .
	manualset3
146321	13	409473	5	NULL	NULL	0	NULL	micro-organism	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The delay observed between admission to hospital and first symptoms , together with the presence of anatomical lesions or physiological disturbances suggesting bacterial invasion by the intestinal route , have led the authors to postulate a nosocomial digestive contamination , probably from water , as suggested by the particular ecology of this micro-organism .
	manualset3
146322	1	409474	5	NULL	NULL	0	NULL	deletions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The deletions of inverted repeat , DPE , and GC-rich regions in P2 had the highest negative impact on this promoter .
	manualset3
146323	2	409474	5	NULL	NULL	0	NULL	inverted repeat 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The deletions of inverted repeat , DPE , and GC-rich regions in P2 had the highest negative impact on this promoter .
	manualset3
146324	3	409474	5	NULL	NULL	0	NULL	DPE 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The deletions of inverted repeat , DPE , and GC-rich regions in P2 had the highest negative impact on this promoter .
	manualset3
146325	4	409474	5	NULL	NULL	0	NULL	GC-rich regions	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The deletions of inverted repeat , DPE , and GC-rich regions in P2 had the highest negative impact on this promoter .
	manualset3
146326	5	409474	5	NULL	NULL	0	NULL	 P2	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The deletions of inverted repeat , DPE , and GC-rich regions in P2 had the highest negative impact on this promoter .
	manualset3
146327	6	409474	5	NULL	NULL	0	NULL	negative impact	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The deletions of inverted repeat , DPE , and GC-rich regions in P2 had the highest negative impact on this promoter .
	manualset3
146328	7	409474	5	NULL	NULL	0	NULL	promoter 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The deletions of inverted repeat , DPE , and GC-rich regions in P2 had the highest negative impact on this promoter .
	manualset3
146329	1	409475	5	NULL	NULL	0	NULL	simple method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple method for determining the lower limit of detection ( LLD ) for personnel dosimetry systems is described .
	manualset3
146330	2	409475	5	NULL	NULL	0	NULL	lower limit of detection ( LLD )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple method for determining the lower limit of detection ( LLD ) for personnel dosimetry systems is described .
	manualset3
146331	3	409475	5	NULL	NULL	0	NULL	personnel dosimetry systems	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple method for determining the lower limit of detection ( LLD ) for personnel dosimetry systems is described .
	manualset3
146332	1	409476	5	NULL	NULL	0	NULL	nitroimidazoles 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The delta ( sol ) H for all the nitroimidazoles is endothermic at pH 2 and 6 but both the macrolides show exothermic behavior , whereas the enthalpy of solution of omeprazole changes from -40.52 to 4.35 kJmol ( -1 ) as the pH changes from 2 to 6 .
	manualset3
146333	2	409476	5	NULL	NULL	0	NULL	pH 2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The delta ( sol ) H for all the nitroimidazoles is endothermic at pH 2 and 6 but both the macrolides show exothermic behavior , whereas the enthalpy of solution of omeprazole changes from -40.52 to 4.35 kJmol ( -1 ) as the pH changes from 2 to 6 .
	manualset3
146334	3	409476	5	NULL	NULL	0	NULL	pH 6	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The delta ( sol ) H for all the nitroimidazoles is endothermic at pH 2 and 6 but both the macrolides show exothermic behavior , whereas the enthalpy of solution of omeprazole changes from -40.52 to 4.35 kJmol ( -1 ) as the pH changes from 2 to 6 .
	manualset3
146335	4	409476	5	NULL	NULL	0	NULL	macrolides 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The delta ( sol ) H for all the nitroimidazoles is endothermic at pH 2 and 6 but both the macrolides show exothermic behavior , whereas the enthalpy of solution of omeprazole changes from -40.52 to 4.35 kJmol ( -1 ) as the pH changes from 2 to 6 .
	manualset3
146336	5	409476	5	NULL	NULL	0	NULL	exothermic behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The delta ( sol ) H for all the nitroimidazoles is endothermic at pH 2 and 6 but both the macrolides show exothermic behavior , whereas the enthalpy of solution of omeprazole changes from -40.52 to 4.35 kJmol ( -1 ) as the pH changes from 2 to 6 .
	manualset3
146337	6	409476	5	NULL	NULL	0	NULL	enthalpy 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The delta ( sol ) H for all the nitroimidazoles is endothermic at pH 2 and 6 but both the macrolides show exothermic behavior , whereas the enthalpy of solution of omeprazole changes from -40.52 to 4.35 kJmol ( -1 ) as the pH changes from 2 to 6 .
	manualset3
146338	7	409476	5	NULL	NULL	0	NULL	solution of omeprazole 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The delta ( sol ) H for all the nitroimidazoles is endothermic at pH 2 and 6 but both the macrolides show exothermic behavior , whereas the enthalpy of solution of omeprazole changes from -40.52 to 4.35 kJmol ( -1 ) as the pH changes from 2 to 6 .
	manualset3
146339	8	409476	5	NULL	NULL	0	NULL	 -40.52 to 4.35 kJmol ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The delta ( sol ) H for all the nitroimidazoles is endothermic at pH 2 and 6 but both the macrolides show exothermic behavior , whereas the enthalpy of solution of omeprazole changes from -40.52 to 4.35 kJmol ( -1 ) as the pH changes from 2 to 6 .
	manualset3
146340	9	409476	5	NULL	NULL	0	NULL	pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The delta ( sol ) H for all the nitroimidazoles is endothermic at pH 2 and 6 but both the macrolides show exothermic behavior , whereas the enthalpy of solution of omeprazole changes from -40.52 to 4.35 kJmol ( -1 ) as the pH changes from 2 to 6 .
	manualset3
146341	10	409476	5	NULL	NULL	0	NULL	2 to 6	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The delta ( sol ) H for all the nitroimidazoles is endothermic at pH 2 and 6 but both the macrolides show exothermic behavior , whereas the enthalpy of solution of omeprazole changes from -40.52 to 4.35 kJmol ( -1 ) as the pH changes from 2 to 6 .
	manualset3
148672	11	409476	5	NULL	NULL	0	NULL	delta ( sol ) H	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The delta ( sol ) H for all the nitroimidazoles is endothermic at pH 2 and 6 but both the macrolides show exothermic behavior , whereas the enthalpy of solution of omeprazole changes from -40.52 to 4.35 kJmol ( -1 ) as the pH changes from 2 to 6 .
	manualset3
146342	1	409477	5	NULL	NULL	0	NULL	demonstration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The demonstration of CKs but not vimentin in the neoplastic cells of a serous superficial ovarian papilloma suggested an origin from the ovarian surface epithelium , while the coexpression of CKs and vimentin in serous papillary and mucinous cystadenomas pointed to a possible origin from the rete ovarii .
	manualset3
146343	2	409477	5	NULL	NULL	0	NULL	CKs 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The demonstration of CKs but not vimentin in the neoplastic cells of a serous superficial ovarian papilloma suggested an origin from the ovarian surface epithelium , while the coexpression of CKs and vimentin in serous papillary and mucinous cystadenomas pointed to a possible origin from the rete ovarii .
	manualset3
146344	3	409477	5	NULL	NULL	0	NULL	vimentin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The demonstration of CKs but not vimentin in the neoplastic cells of a serous superficial ovarian papilloma suggested an origin from the ovarian surface epithelium , while the coexpression of CKs and vimentin in serous papillary and mucinous cystadenomas pointed to a possible origin from the rete ovarii .
	manualset3
146345	4	409477	5	NULL	NULL	0	NULL	neoplastic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The demonstration of CKs but not vimentin in the neoplastic cells of a serous superficial ovarian papilloma suggested an origin from the ovarian surface epithelium , while the coexpression of CKs and vimentin in serous papillary and mucinous cystadenomas pointed to a possible origin from the rete ovarii .
	manualset3
146346	5	409477	5	NULL	NULL	0	NULL	serous superficial ovarian papilloma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The demonstration of CKs but not vimentin in the neoplastic cells of a serous superficial ovarian papilloma suggested an origin from the ovarian surface epithelium , while the coexpression of CKs and vimentin in serous papillary and mucinous cystadenomas pointed to a possible origin from the rete ovarii .
	manualset3
146347	6	409477	5	NULL	NULL	0	NULL	origin 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The demonstration of CKs but not vimentin in the neoplastic cells of a serous superficial ovarian papilloma suggested an origin from the ovarian surface epithelium , while the coexpression of CKs and vimentin in serous papillary and mucinous cystadenomas pointed to a possible origin from the rete ovarii .
	manualset3
146348	7	409477	5	NULL	NULL	0	NULL	ovarian surface epithelium	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The demonstration of CKs but not vimentin in the neoplastic cells of a serous superficial ovarian papilloma suggested an origin from the ovarian surface epithelium , while the coexpression of CKs and vimentin in serous papillary and mucinous cystadenomas pointed to a possible origin from the rete ovarii .
	manualset3
146349	8	409477	5	NULL	NULL	0	NULL	coexpression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The demonstration of CKs but not vimentin in the neoplastic cells of a serous superficial ovarian papilloma suggested an origin from the ovarian surface epithelium , while the coexpression of CKs and vimentin in serous papillary and mucinous cystadenomas pointed to a possible origin from the rete ovarii .
	manualset3
146350	9	409477	5	NULL	NULL	0	NULL	CKs 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The demonstration of CKs but not vimentin in the neoplastic cells of a serous superficial ovarian papilloma suggested an origin from the ovarian surface epithelium , while the coexpression of CKs and vimentin in serous papillary and mucinous cystadenomas pointed to a possible origin from the rete ovarii .
	manualset3
146351	10	409477	5	NULL	NULL	0	NULL	vimentin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The demonstration of CKs but not vimentin in the neoplastic cells of a serous superficial ovarian papilloma suggested an origin from the ovarian surface epithelium , while the coexpression of CKs and vimentin in serous papillary and mucinous cystadenomas pointed to a possible origin from the rete ovarii .
	manualset3
146352	11	409477	5	NULL	NULL	0	NULL	serous papillary	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The demonstration of CKs but not vimentin in the neoplastic cells of a serous superficial ovarian papilloma suggested an origin from the ovarian surface epithelium , while the coexpression of CKs and vimentin in serous papillary and mucinous cystadenomas pointed to a possible origin from the rete ovarii .
	manualset3
146353	12	409477	5	NULL	NULL	0	NULL	mucinous cystadenomas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The demonstration of CKs but not vimentin in the neoplastic cells of a serous superficial ovarian papilloma suggested an origin from the ovarian surface epithelium , while the coexpression of CKs and vimentin in serous papillary and mucinous cystadenomas pointed to a possible origin from the rete ovarii .
	manualset3
146354	13	409477	5	NULL	NULL	0	NULL	origin 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The demonstration of CKs but not vimentin in the neoplastic cells of a serous superficial ovarian papilloma suggested an origin from the ovarian surface epithelium , while the coexpression of CKs and vimentin in serous papillary and mucinous cystadenomas pointed to a possible origin from the rete ovarii .
	manualset3
146355	14	409477	5	NULL	NULL	0	NULL	rete ovarii	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The demonstration of CKs but not vimentin in the neoplastic cells of a serous superficial ovarian papilloma suggested an origin from the ovarian surface epithelium , while the coexpression of CKs and vimentin in serous papillary and mucinous cystadenomas pointed to a possible origin from the rete ovarii .
	manualset3
146356	1	409478	5	NULL	NULL	0	NULL	demonstration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The demonstration of recent myocardial injury : a simple method suitable for routine use .
	manualset3
146357	2	409478	5	NULL	NULL	0	NULL	myocardial injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The demonstration of recent myocardial injury : a simple method suitable for routine use .
	manualset3
146358	3	409478	5	NULL	NULL	NULL	NULL	simple method	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The demonstration of recent myocardial injury : a simple method suitable for routine use .
	manualset3
146359	4	409478	5	NULL	NULL	0	NULL	routine use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The demonstration of recent myocardial injury : a simple method suitable for routine use .
	manualset3
146360	1	409479	5	NULL	NULL	0	NULL	demonstration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The demonstration that replication-impaired , poorly competitive progenitor cell pools can promote tumorigenesis provides a new rationale for links between tumorigenesis and common human conditions of impaired DNA replication such as dietary folate deficiency , chemotherapeutics targeting dNTP synthesis , and polymorphisms in genes important for DNA metabolism .
	manualset3
146361	2	409479	5	NULL	NULL	0	NULL	progenitor cell pools	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The demonstration that replication-impaired , poorly competitive progenitor cell pools can promote tumorigenesis provides a new rationale for links between tumorigenesis and common human conditions of impaired DNA replication such as dietary folate deficiency , chemotherapeutics targeting dNTP synthesis , and polymorphisms in genes important for DNA metabolism .
	manualset3
146362	3	409479	5	NULL	NULL	0	NULL	tumorigenesis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The demonstration that replication-impaired , poorly competitive progenitor cell pools can promote tumorigenesis provides a new rationale for links between tumorigenesis and common human conditions of impaired DNA replication such as dietary folate deficiency , chemotherapeutics targeting dNTP synthesis , and polymorphisms in genes important for DNA metabolism .
	manualset3
146363	4	409479	5	NULL	NULL	0	NULL	links 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The demonstration that replication-impaired , poorly competitive progenitor cell pools can promote tumorigenesis provides a new rationale for links between tumorigenesis and common human conditions of impaired DNA replication such as dietary folate deficiency , chemotherapeutics targeting dNTP synthesis , and polymorphisms in genes important for DNA metabolism .
	manualset3
146364	5	409479	5	NULL	NULL	0	NULL	tumorigenesis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The demonstration that replication-impaired , poorly competitive progenitor cell pools can promote tumorigenesis provides a new rationale for links between tumorigenesis and common human conditions of impaired DNA replication such as dietary folate deficiency , chemotherapeutics targeting dNTP synthesis , and polymorphisms in genes important for DNA metabolism .
	manualset3
146365	6	409479	5	NULL	NULL	0	NULL	common human conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The demonstration that replication-impaired , poorly competitive progenitor cell pools can promote tumorigenesis provides a new rationale for links between tumorigenesis and common human conditions of impaired DNA replication such as dietary folate deficiency , chemotherapeutics targeting dNTP synthesis , and polymorphisms in genes important for DNA metabolism .
	manualset3
146366	7	409479	5	NULL	NULL	0	NULL	impaired DNA replication	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The demonstration that replication-impaired , poorly competitive progenitor cell pools can promote tumorigenesis provides a new rationale for links between tumorigenesis and common human conditions of impaired DNA replication such as dietary folate deficiency , chemotherapeutics targeting dNTP synthesis , and polymorphisms in genes important for DNA metabolism .
	manualset3
146367	8	409479	5	NULL	NULL	0	NULL	dietary folate deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The demonstration that replication-impaired , poorly competitive progenitor cell pools can promote tumorigenesis provides a new rationale for links between tumorigenesis and common human conditions of impaired DNA replication such as dietary folate deficiency , chemotherapeutics targeting dNTP synthesis , and polymorphisms in genes important for DNA metabolism .
	manualset3
146368	9	409479	5	NULL	NULL	NULL	NULL	chemotherapeutics 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The demonstration that replication-impaired , poorly competitive progenitor cell pools can promote tumorigenesis provides a new rationale for links between tumorigenesis and common human conditions of impaired DNA replication such as dietary folate deficiency , chemotherapeutics targeting dNTP synthesis , and polymorphisms in genes important for DNA metabolism .
	manualset3
146369	10	409479	5	NULL	NULL	0	NULL	dNTP synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The demonstration that replication-impaired , poorly competitive progenitor cell pools can promote tumorigenesis provides a new rationale for links between tumorigenesis and common human conditions of impaired DNA replication such as dietary folate deficiency , chemotherapeutics targeting dNTP synthesis , and polymorphisms in genes important for DNA metabolism .
	manualset3
146370	11	409479	5	NULL	NULL	0	NULL	polymorphisms 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The demonstration that replication-impaired , poorly competitive progenitor cell pools can promote tumorigenesis provides a new rationale for links between tumorigenesis and common human conditions of impaired DNA replication such as dietary folate deficiency , chemotherapeutics targeting dNTP synthesis , and polymorphisms in genes important for DNA metabolism .
	manualset3
146371	12	409479	5	NULL	NULL	0	NULL	genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The demonstration that replication-impaired , poorly competitive progenitor cell pools can promote tumorigenesis provides a new rationale for links between tumorigenesis and common human conditions of impaired DNA replication such as dietary folate deficiency , chemotherapeutics targeting dNTP synthesis , and polymorphisms in genes important for DNA metabolism .
	manualset3
146372	13	409479	5	NULL	NULL	0	NULL	DNA metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The demonstration that replication-impaired , poorly competitive progenitor cell pools can promote tumorigenesis provides a new rationale for links between tumorigenesis and common human conditions of impaired DNA replication such as dietary folate deficiency , chemotherapeutics targeting dNTP synthesis , and polymorphisms in genes important for DNA metabolism .
	manualset3
148673	14	409479	5	NULL	NULL	0	NULL	rationale 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The demonstration that replication-impaired , poorly competitive progenitor cell pools can promote tumorigenesis provides a new rationale for links between tumorigenesis and common human conditions of impaired DNA replication such as dietary folate deficiency , chemotherapeutics targeting dNTP synthesis , and polymorphisms in genes important for DNA metabolism .
	manualset3
146373	1	409480	5	NULL	NULL	0	NULL	densities 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The densities of the HCC and liver were decreased and increased during scanning , respectively .
	manualset3
146374	2	409480	5	NULL	NULL	0	NULL	HCC 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The densities of the HCC and liver were decreased and increased during scanning , respectively .
	manualset3
146375	3	409480	5	NULL	NULL	0	NULL	liver 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The densities of the HCC and liver were decreased and increased during scanning , respectively .
	manualset3
146376	4	409480	5	NULL	NULL	0	NULL	scanning 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The densities of the HCC and liver were decreased and increased during scanning , respectively .
	manualset3
146377	1	409481	5	NULL	NULL	0	NULL	depletion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The depletion of ATP and the consequent increase of electron density or c-value of the fixed anionic groups turns NaCl ( ineffective in causing swelling of normal tissues ) into a fully effective agent for causing swelling of the injured tissues .
	manualset3
146378	2	409481	5	NULL	NULL	0	NULL	ATP 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The depletion of ATP and the consequent increase of electron density or c-value of the fixed anionic groups turns NaCl ( ineffective in causing swelling of normal tissues ) into a fully effective agent for causing swelling of the injured tissues .
	manualset3
146379	3	409481	5	NULL	NULL	0	NULL	electron density	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The depletion of ATP and the consequent increase of electron density or c-value of the fixed anionic groups turns NaCl ( ineffective in causing swelling of normal tissues ) into a fully effective agent for causing swelling of the injured tissues .
	manualset3
146380	4	409481	5	NULL	NULL	0	NULL	c-value 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The depletion of ATP and the consequent increase of electron density or c-value of the fixed anionic groups turns NaCl ( ineffective in causing swelling of normal tissues ) into a fully effective agent for causing swelling of the injured tissues .
	manualset3
146381	5	409481	5	NULL	NULL	0	NULL	fixed anionic groups	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The depletion of ATP and the consequent increase of electron density or c-value of the fixed anionic groups turns NaCl ( ineffective in causing swelling of normal tissues ) into a fully effective agent for causing swelling of the injured tissues .
	manualset3
146382	6	409481	5	NULL	NULL	0	NULL	NaCl 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The depletion of ATP and the consequent increase of electron density or c-value of the fixed anionic groups turns NaCl ( ineffective in causing swelling of normal tissues ) into a fully effective agent for causing swelling of the injured tissues .
	manualset3
146383	7	409481	5	NULL	NULL	0	NULL	swelling 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The depletion of ATP and the consequent increase of electron density or c-value of the fixed anionic groups turns NaCl ( ineffective in causing swelling of normal tissues ) into a fully effective agent for causing swelling of the injured tissues .
	manualset3
146384	8	409481	5	NULL	NULL	0	NULL	normal tissues 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The depletion of ATP and the consequent increase of electron density or c-value of the fixed anionic groups turns NaCl ( ineffective in causing swelling of normal tissues ) into a fully effective agent for causing swelling of the injured tissues .
	manualset3
146385	9	409481	5	NULL	NULL	0	NULL	effective agent	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The depletion of ATP and the consequent increase of electron density or c-value of the fixed anionic groups turns NaCl ( ineffective in causing swelling of normal tissues ) into a fully effective agent for causing swelling of the injured tissues .
	manualset3
146386	10	409481	5	NULL	NULL	0	NULL	swelling 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The depletion of ATP and the consequent increase of electron density or c-value of the fixed anionic groups turns NaCl ( ineffective in causing swelling of normal tissues ) into a fully effective agent for causing swelling of the injured tissues .
	manualset3
146387	11	409481	5	NULL	NULL	0	NULL	injured tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The depletion of ATP and the consequent increase of electron density or c-value of the fixed anionic groups turns NaCl ( ineffective in causing swelling of normal tissues ) into a fully effective agent for causing swelling of the injured tissues .
	manualset3
146388	1	409482	5	NULL	NULL	0	NULL	simple method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple method for quantifying nosocomial infection and colonization with multidrug-resistant organisms is described .
	manualset3
146389	2	409482	5	NULL	NULL	0	NULL	nosocomial infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple method for quantifying nosocomial infection and colonization with multidrug-resistant organisms is described .
	manualset3
146390	3	409482	5	NULL	NULL	0	NULL	colonization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple method for quantifying nosocomial infection and colonization with multidrug-resistant organisms is described .
	manualset3
146391	4	409482	5	NULL	NULL	0	NULL	multidrug-resistant organisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple method for quantifying nosocomial infection and colonization with multidrug-resistant organisms is described .
	manualset3
146392	1	409483	5	NULL	NULL	0	NULL	LNC reactivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The depressed LNC reactivity to BP in Con A-treated animals was not increased when nylon wool adherent cells were removed , whereas there was a significant increase in unsuppressed animals .
	manualset3
146393	2	409483	5	NULL	NULL	0	NULL	BP 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The depressed LNC reactivity to BP in Con A-treated animals was not increased when nylon wool adherent cells were removed , whereas there was a significant increase in unsuppressed animals .
	manualset3
146394	3	409483	5	NULL	NULL	0	NULL	Con A-treated animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The depressed LNC reactivity to BP in Con A-treated animals was not increased when nylon wool adherent cells were removed , whereas there was a significant increase in unsuppressed animals .
	manualset3
146395	4	409483	5	NULL	NULL	0	NULL	nylon wool adherent cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The depressed LNC reactivity to BP in Con A-treated animals was not increased when nylon wool adherent cells were removed , whereas there was a significant increase in unsuppressed animals .
	manualset3
146396	5	409483	5	NULL	NULL	0	NULL	unsuppressed animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The depressed LNC reactivity to BP in Con A-treated animals was not increased when nylon wool adherent cells were removed , whereas there was a significant increase in unsuppressed animals .
	manualset3
146397	1	409484	5	NULL	NULL	0	NULL	derivation cohort 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The derivation cohort included 339 patients admitted to a large hospital in Rome during 2008 , with ( n = 113 ) or without ( n = 226 ) culture positivity for ESBL-producing Escherichia coli , Klebsiella spp. , or Proteus mirabilis within 48 h after admission .
	manualset3
146398	2	409484	5	NULL	NULL	0	NULL	339 patients	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The derivation cohort included 339 patients admitted to a large hospital in Rome during 2008 , with ( n = 113 ) or without ( n = 226 ) culture positivity for ESBL-producing Escherichia coli , Klebsiella spp. , or Proteus mirabilis within 48 h after admission .
	manualset3
146399	3	409484	5	NULL	NULL	0	NULL	hospital 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The derivation cohort included 339 patients admitted to a large hospital in Rome during 2008 , with ( n = 113 ) or without ( n = 226 ) culture positivity for ESBL-producing Escherichia coli , Klebsiella spp. , or Proteus mirabilis within 48 h after admission .
	manualset3
146400	4	409484	5	NULL	NULL	0	NULL	Rome 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The derivation cohort included 339 patients admitted to a large hospital in Rome during 2008 , with ( n = 113 ) or without ( n = 226 ) culture positivity for ESBL-producing Escherichia coli , Klebsiella spp. , or Proteus mirabilis within 48 h after admission .
	manualset3
146401	5	409484	5	NULL	NULL	0	NULL	2008 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	The derivation cohort included 339 patients admitted to a large hospital in Rome during 2008 , with ( n = 113 ) or without ( n = 226 ) culture positivity for ESBL-producing Escherichia coli , Klebsiella spp. , or Proteus mirabilis within 48 h after admission .
	manualset3
146402	6	409484	5	NULL	NULL	0	NULL	 n = 113	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The derivation cohort included 339 patients admitted to a large hospital in Rome during 2008 , with ( n = 113 ) or without ( n = 226 ) culture positivity for ESBL-producing Escherichia coli , Klebsiella spp. , or Proteus mirabilis within 48 h after admission .
	manualset3
146403	7	409484	5	NULL	NULL	0	NULL	n = 226	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The derivation cohort included 339 patients admitted to a large hospital in Rome during 2008 , with ( n = 113 ) or without ( n = 226 ) culture positivity for ESBL-producing Escherichia coli , Klebsiella spp. , or Proteus mirabilis within 48 h after admission .
	manualset3
146404	8	409484	5	NULL	NULL	0	NULL	ESBL-producing Escherichia coli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The derivation cohort included 339 patients admitted to a large hospital in Rome during 2008 , with ( n = 113 ) or without ( n = 226 ) culture positivity for ESBL-producing Escherichia coli , Klebsiella spp. , or Proteus mirabilis within 48 h after admission .
	manualset3
146405	9	409484	5	NULL	NULL	0	NULL	Klebsiella spp.	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The derivation cohort included 339 patients admitted to a large hospital in Rome during 2008 , with ( n = 113 ) or without ( n = 226 ) culture positivity for ESBL-producing Escherichia coli , Klebsiella spp. , or Proteus mirabilis within 48 h after admission .
	manualset3
146406	10	409484	5	NULL	NULL	0	NULL	Proteus mirabilis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The derivation cohort included 339 patients admitted to a large hospital in Rome during 2008 , with ( n = 113 ) or without ( n = 226 ) culture positivity for ESBL-producing Escherichia coli , Klebsiella spp. , or Proteus mirabilis within 48 h after admission .
	manualset3
146407	11	409484	5	NULL	NULL	0	NULL	48 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The derivation cohort included 339 patients admitted to a large hospital in Rome during 2008 , with ( n = 113 ) or without ( n = 226 ) culture positivity for ESBL-producing Escherichia coli , Klebsiella spp. , or Proteus mirabilis within 48 h after admission .
	manualset3
146408	12	409484	5	NULL	NULL	0	NULL	admission 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The derivation cohort included 339 patients admitted to a large hospital in Rome during 2008 , with ( n = 113 ) or without ( n = 226 ) culture positivity for ESBL-producing Escherichia coli , Klebsiella spp. , or Proteus mirabilis within 48 h after admission .
	manualset3
146409	1	409485	5	NULL	NULL	0	NULL	derived cell envelopes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The derived cell envelopes contained 61 % protein , 3 % ash , 23 % lipid , and 1 % phosphorus .
	manualset3
146410	2	409485	5	NULL	NULL	0	NULL	61 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The derived cell envelopes contained 61 % protein , 3 % ash , 23 % lipid , and 1 % phosphorus .
	manualset3
146411	3	409485	5	NULL	NULL	0	NULL	protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The derived cell envelopes contained 61 % protein , 3 % ash , 23 % lipid , and 1 % phosphorus .
	manualset3
146412	4	409485	5	NULL	NULL	0	NULL	3 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The derived cell envelopes contained 61 % protein , 3 % ash , 23 % lipid , and 1 % phosphorus .
	manualset3
146413	5	409485	5	NULL	NULL	0	NULL	ash 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The derived cell envelopes contained 61 % protein , 3 % ash , 23 % lipid , and 1 % phosphorus .
	manualset3
146414	6	409485	5	NULL	NULL	0	NULL	23 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The derived cell envelopes contained 61 % protein , 3 % ash , 23 % lipid , and 1 % phosphorus .
	manualset3
146415	7	409485	5	NULL	NULL	0	NULL	lipid 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The derived cell envelopes contained 61 % protein , 3 % ash , 23 % lipid , and 1 % phosphorus .
	manualset3
146416	8	409485	5	NULL	NULL	0	NULL	 1 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The derived cell envelopes contained 61 % protein , 3 % ash , 23 % lipid , and 1 % phosphorus .
	manualset3
146417	9	409485	5	NULL	NULL	0	NULL	phosphorus 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The derived cell envelopes contained 61 % protein , 3 % ash , 23 % lipid , and 1 % phosphorus .
	manualset3
146418	1	409486	5	NULL	NULL	0	NULL	dermal and endochondral bones of the girdle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The dermal and endochondral bones of the girdle form immobile joints with neighboring girdle elements ; however , the cellular organization and growth pattern of the scapula and coracoid closely resemble those of a long bone .
	manualset3
146419	2	409486	5	NULL	NULL	0	NULL	immobile joints	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The dermal and endochondral bones of the girdle form immobile joints with neighboring girdle elements ; however , the cellular organization and growth pattern of the scapula and coracoid closely resemble those of a long bone .
	manualset3
146420	3	409486	5	NULL	NULL	0	NULL	neighboring girdle elements	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The dermal and endochondral bones of the girdle form immobile joints with neighboring girdle elements ; however , the cellular organization and growth pattern of the scapula and coracoid closely resemble those of a long bone .
	manualset3
146421	4	409486	5	NULL	NULL	0	NULL	cellular organization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The dermal and endochondral bones of the girdle form immobile joints with neighboring girdle elements ; however , the cellular organization and growth pattern of the scapula and coracoid closely resemble those of a long bone .
	manualset3
146422	5	409486	5	NULL	NULL	0	NULL	growth pattern	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The dermal and endochondral bones of the girdle form immobile joints with neighboring girdle elements ; however , the cellular organization and growth pattern of the scapula and coracoid closely resemble those of a long bone .
	manualset3
146423	6	409486	5	NULL	NULL	0	NULL	scapula 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The dermal and endochondral bones of the girdle form immobile joints with neighboring girdle elements ; however , the cellular organization and growth pattern of the scapula and coracoid closely resemble those of a long bone .
	manualset3
146424	7	409486	5	NULL	NULL	0	NULL	coracoid 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The dermal and endochondral bones of the girdle form immobile joints with neighboring girdle elements ; however , the cellular organization and growth pattern of the scapula and coracoid closely resemble those of a long bone .
	manualset3
146425	8	409486	5	NULL	NULL	0	NULL	long bone	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The dermal and endochondral bones of the girdle form immobile joints with neighboring girdle elements ; however , the cellular organization and growth pattern of the scapula and coracoid closely resemble those of a long bone .
	manualset3
146426	1	409487	5	NULL	NULL	0	NULL	changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The described changes in the bone blood flow and mineral content under the given experimental conditions suggest a relation in the regulations of both processes , a possible association with resorption of bone , and the importance of the circulation of blood in the metabolism of bone tissue .
	manualset3
146427	2	409487	5	NULL	NULL	0	NULL	bone blood flow	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The described changes in the bone blood flow and mineral content under the given experimental conditions suggest a relation in the regulations of both processes , a possible association with resorption of bone , and the importance of the circulation of blood in the metabolism of bone tissue .
	manualset3
146428	3	409487	5	NULL	NULL	0	NULL	mineral content 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The described changes in the bone blood flow and mineral content under the given experimental conditions suggest a relation in the regulations of both processes , a possible association with resorption of bone , and the importance of the circulation of blood in the metabolism of bone tissue .
	manualset3
146429	4	409487	5	NULL	NULL	0	NULL	experimental conditions 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The described changes in the bone blood flow and mineral content under the given experimental conditions suggest a relation in the regulations of both processes , a possible association with resorption of bone , and the importance of the circulation of blood in the metabolism of bone tissue .
	manualset3
146430	5	409487	5	NULL	NULL	0	NULL	relation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The described changes in the bone blood flow and mineral content under the given experimental conditions suggest a relation in the regulations of both processes , a possible association with resorption of bone , and the importance of the circulation of blood in the metabolism of bone tissue .
	manualset3
146431	6	409487	5	NULL	NULL	0	NULL	regulations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The described changes in the bone blood flow and mineral content under the given experimental conditions suggest a relation in the regulations of both processes , a possible association with resorption of bone , and the importance of the circulation of blood in the metabolism of bone tissue .
	manualset3
146432	7	409487	5	NULL	NULL	0	NULL	processes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The described changes in the bone blood flow and mineral content under the given experimental conditions suggest a relation in the regulations of both processes , a possible association with resorption of bone , and the importance of the circulation of blood in the metabolism of bone tissue .
	manualset3
146435	8	409487	5	NULL	NULL	0	NULL	possible association	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The described changes in the bone blood flow and mineral content under the given experimental conditions suggest a relation in the regulations of both processes , a possible association with resorption of bone , and the importance of the circulation of blood in the metabolism of bone tissue .
	manualset3
146436	9	409487	5	NULL	NULL	NULL	NULL	resorption of bone	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The described changes in the bone blood flow and mineral content under the given experimental conditions suggest a relation in the regulations of both processes , a possible association with resorption of bone , and the importance of the circulation of blood in the metabolism of bone tissue .
	manualset3
146437	10	409487	5	NULL	NULL	NULL	NULL	circulation of blood	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The described changes in the bone blood flow and mineral content under the given experimental conditions suggest a relation in the regulations of both processes , a possible association with resorption of bone , and the importance of the circulation of blood in the metabolism of bone tissue .
	manualset3
146438	11	409487	5	NULL	NULL	0	NULL	metabolism of bone tissue	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The described changes in the bone blood flow and mineral content under the given experimental conditions suggest a relation in the regulations of both processes , a possible association with resorption of bone , and the importance of the circulation of blood in the metabolism of bone tissue .
	manualset3
146439	1	409488	5	NULL	NULL	0	NULL	design 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The design and synthesis of mimetics of peptide beta-turns .
	manualset3
146440	2	409488	5	NULL	NULL	0	NULL	synthesis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The design and synthesis of mimetics of peptide beta-turns .
	manualset3
146441	3	409488	5	NULL	NULL	0	NULL	peptide beta-turns	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The design and synthesis of mimetics of peptide beta-turns .
	manualset3
146442	1	409489	5	NULL	NULL	0	NULL	design 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The design of polymer microcarrier surfaces for enhanced cell growth .
	manualset3
146443	2	409489	5	NULL	NULL	0	NULL	polymer microcarrier surfaces	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The design of polymer microcarrier surfaces for enhanced cell growth .
	manualset3
146444	3	409489	5	NULL	NULL	0	NULL	enhanced cell growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The design of polymer microcarrier surfaces for enhanced cell growth .
	manualset3
146445	1	409490	5	NULL	NULL	0	NULL	design 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The design of the NIMH-sponsored Clinical Antipsychotic Trials of Intervention Effectiveness ( CATIE ) Schizophrenia Trial was driven by a need to understand the efficacy and safety differences between atypical antipsychotics , and between atypical and typical antipsychotics .
	manualset3
146446	2	409490	5	NULL	NULL	NULL	NULL	NIMH-sponsored Clinical Antipsychotic Trials of Intervention Effectiveness ( CATIE ) Schizophrenia Trial 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The design of the NIMH-sponsored Clinical Antipsychotic Trials of Intervention Effectiveness ( CATIE ) Schizophrenia Trial was driven by a need to understand the efficacy and safety differences between atypical antipsychotics , and between atypical and typical antipsychotics .
	manualset3
146447	3	409490	5	NULL	NULL	0	NULL	efficacy 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The design of the NIMH-sponsored Clinical Antipsychotic Trials of Intervention Effectiveness ( CATIE ) Schizophrenia Trial was driven by a need to understand the efficacy and safety differences between atypical antipsychotics , and between atypical and typical antipsychotics .
	manualset3
146448	4	409490	5	NULL	NULL	0	NULL	safety differences 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The design of the NIMH-sponsored Clinical Antipsychotic Trials of Intervention Effectiveness ( CATIE ) Schizophrenia Trial was driven by a need to understand the efficacy and safety differences between atypical antipsychotics , and between atypical and typical antipsychotics .
	manualset3
146449	5	409490	5	NULL	NULL	0	NULL	atypical antipsychotics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The design of the NIMH-sponsored Clinical Antipsychotic Trials of Intervention Effectiveness ( CATIE ) Schizophrenia Trial was driven by a need to understand the efficacy and safety differences between atypical antipsychotics , and between atypical and typical antipsychotics .
	manualset3
146450	6	409490	5	NULL	NULL	0	NULL	atypical antipsychotics 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The design of the NIMH-sponsored Clinical Antipsychotic Trials of Intervention Effectiveness ( CATIE ) Schizophrenia Trial was driven by a need to understand the efficacy and safety differences between atypical antipsychotics , and between atypical and typical antipsychotics .
	manualset3
146451	7	409490	5	NULL	NULL	0	NULL	typical antipsychotics 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The design of the NIMH-sponsored Clinical Antipsychotic Trials of Intervention Effectiveness ( CATIE ) Schizophrenia Trial was driven by a need to understand the efficacy and safety differences between atypical antipsychotics , and between atypical and typical antipsychotics .
	manualset3
146452	1	409491	5	NULL	NULL	0	NULL	mushroom body	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple mushroom body in an African scarabid beetle .
	manualset3
146453	2	409491	5	NULL	NULL	0	NULL	African scarabid beetle	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple mushroom body in an African scarabid beetle .
	manualset3
146454	1	409492	5	NULL	NULL	0	NULL	investigations 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The detailed investigations for the ground state and the pi -- ) pi * excited state of ethene clarified three aspects about DFT and TDDFT methods : First , the DFT methods included electron correlation effects by directly changing MO energies and MO electron density distributions .
	manualset3
146455	2	409492	5	NULL	NULL	0	NULL	ground state 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The detailed investigations for the ground state and the pi -- ) pi * excited state of ethene clarified three aspects about DFT and TDDFT methods : First , the DFT methods included electron correlation effects by directly changing MO energies and MO electron density distributions .
	manualset3
146456	3	409492	5	NULL	NULL	0	NULL	 pi -- ) pi * excited state 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The detailed investigations for the ground state and the pi -- ) pi * excited state of ethene clarified three aspects about DFT and TDDFT methods : First , the DFT methods included electron correlation effects by directly changing MO energies and MO electron density distributions .
	manualset3
146457	4	409492	5	NULL	NULL	0	NULL	ethene 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The detailed investigations for the ground state and the pi -- ) pi * excited state of ethene clarified three aspects about DFT and TDDFT methods : First , the DFT methods included electron correlation effects by directly changing MO energies and MO electron density distributions .
	manualset3
146458	5	409492	5	NULL	NULL	0	NULL	three aspects	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The detailed investigations for the ground state and the pi -- ) pi * excited state of ethene clarified three aspects about DFT and TDDFT methods : First , the DFT methods included electron correlation effects by directly changing MO energies and MO electron density distributions .
	manualset3
146459	6	409492	5	NULL	NULL	0	NULL	DFT method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The detailed investigations for the ground state and the pi -- ) pi * excited state of ethene clarified three aspects about DFT and TDDFT methods : First , the DFT methods included electron correlation effects by directly changing MO energies and MO electron density distributions .
	manualset3
146460	7	409492	5	NULL	NULL	0	NULL	TDDFT method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The detailed investigations for the ground state and the pi -- ) pi * excited state of ethene clarified three aspects about DFT and TDDFT methods : First , the DFT methods included electron correlation effects by directly changing MO energies and MO electron density distributions .
	manualset3
146461	8	409492	5	NULL	NULL	0	NULL	DFT method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The detailed investigations for the ground state and the pi -- ) pi * excited state of ethene clarified three aspects about DFT and TDDFT methods : First , the DFT methods included electron correlation effects by directly changing MO energies and MO electron density distributions .
	manualset3
146462	9	409492	5	NULL	NULL	0	NULL	electron correlation effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The detailed investigations for the ground state and the pi -- ) pi * excited state of ethene clarified three aspects about DFT and TDDFT methods : First , the DFT methods included electron correlation effects by directly changing MO energies and MO electron density distributions .
	manualset3
146463	10	409492	5	NULL	NULL	0	NULL	MO energies	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The detailed investigations for the ground state and the pi -- ) pi * excited state of ethene clarified three aspects about DFT and TDDFT methods : First , the DFT methods included electron correlation effects by directly changing MO energies and MO electron density distributions .
	manualset3
146464	11	409492	5	NULL	NULL	0	NULL	MO electron density distributions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The detailed investigations for the ground state and the pi -- ) pi * excited state of ethene clarified three aspects about DFT and TDDFT methods : First , the DFT methods included electron correlation effects by directly changing MO energies and MO electron density distributions .
	manualset3
146465	1	409493	5	NULL	NULL	0	NULL	detection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection from human skin of the active ingredients from ointments is reported together with the detection of ibuprofen metabolites in human urine .
	manualset3
146466	2	409493	5	NULL	NULL	0	NULL	human skin	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection from human skin of the active ingredients from ointments is reported together with the detection of ibuprofen metabolites in human urine .
	manualset3
146467	3	409493	5	NULL	NULL	0	NULL	active ingredients	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection from human skin of the active ingredients from ointments is reported together with the detection of ibuprofen metabolites in human urine .
	manualset3
146468	4	409493	5	NULL	NULL	0	NULL	ointments 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection from human skin of the active ingredients from ointments is reported together with the detection of ibuprofen metabolites in human urine .
	manualset3
146469	5	409493	5	NULL	NULL	0	NULL	detection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection from human skin of the active ingredients from ointments is reported together with the detection of ibuprofen metabolites in human urine .
	manualset3
146470	6	409493	5	NULL	NULL	0	NULL	ibuprofen metabolites	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection from human skin of the active ingredients from ointments is reported together with the detection of ibuprofen metabolites in human urine .
	manualset3
146471	7	409493	5	NULL	NULL	0	NULL	human urine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection from human skin of the active ingredients from ointments is reported together with the detection of ibuprofen metabolites in human urine .
	manualset3
146472	1	409494	5	NULL	NULL	0	NULL	detection limit	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection limit of dextromethorphan is 10 ng .
	manualset3
146473	2	409494	5	NULL	NULL	0	NULL	dextromethorphan 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection limit of dextromethorphan is 10 ng .
	manualset3
146474	3	409494	5	NULL	NULL	0	NULL	10 ng	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection limit of dextromethorphan is 10 ng .
	manualset3
146475	1	409495	5	NULL	NULL	0	NULL	detection limits	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection limits ( k = 3 , N = 11 ) were 4.6 microg L ( -1 ) for silver ( I ) and 15.3 microg L ( -1 ) for lead ( II ) .
	manualset3
146476	2	409495	5	NULL	NULL	0	NULL	k = 3 , N = 11	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection limits ( k = 3 , N = 11 ) were 4.6 microg L ( -1 ) for silver ( I ) and 15.3 microg L ( -1 ) for lead ( II ) .
	manualset3
146477	3	409495	5	NULL	NULL	0	NULL	4.6 microg L ( -1 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection limits ( k = 3 , N = 11 ) were 4.6 microg L ( -1 ) for silver ( I ) and 15.3 microg L ( -1 ) for lead ( II ) .
	manualset3
146478	4	409495	5	NULL	NULL	0	NULL	silver ( I )	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection limits ( k = 3 , N = 11 ) were 4.6 microg L ( -1 ) for silver ( I ) and 15.3 microg L ( -1 ) for lead ( II ) .
	manualset3
146479	5	409495	5	NULL	NULL	0	NULL	15.3 microg L ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection limits ( k = 3 , N = 11 ) were 4.6 microg L ( -1 ) for silver ( I ) and 15.3 microg L ( -1 ) for lead ( II ) .
	manualset3
146480	6	409495	5	NULL	NULL	0	NULL	lead ( II )	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection limits ( k = 3 , N = 11 ) were 4.6 microg L ( -1 ) for silver ( I ) and 15.3 microg L ( -1 ) for lead ( II ) .
	manualset3
146481	1	409496	5	NULL	NULL	0	NULL	detection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection of DNA by PCR was the most useful test especially in untreated patients , with a sensitivity of 62 % overall , 81 % in untreated patients and only 20 % in treated patients .
	manualset3
146482	2	409496	5	NULL	NULL	0	NULL	DNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection of DNA by PCR was the most useful test especially in untreated patients , with a sensitivity of 62 % overall , 81 % in untreated patients and only 20 % in treated patients .
	manualset3
146483	3	409496	5	NULL	NULL	0	NULL	PCR 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection of DNA by PCR was the most useful test especially in untreated patients , with a sensitivity of 62 % overall , 81 % in untreated patients and only 20 % in treated patients .
	manualset3
146484	4	409496	5	NULL	NULL	0	NULL	useful test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection of DNA by PCR was the most useful test especially in untreated patients , with a sensitivity of 62 % overall , 81 % in untreated patients and only 20 % in treated patients .
	manualset3
146485	5	409496	5	NULL	NULL	0	NULL	untreated patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection of DNA by PCR was the most useful test especially in untreated patients , with a sensitivity of 62 % overall , 81 % in untreated patients and only 20 % in treated patients .
	manualset3
146486	6	409496	5	NULL	NULL	0	NULL	sensitivity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection of DNA by PCR was the most useful test especially in untreated patients , with a sensitivity of 62 % overall , 81 % in untreated patients and only 20 % in treated patients .
	manualset3
146487	7	409496	5	NULL	NULL	0	NULL	62 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection of DNA by PCR was the most useful test especially in untreated patients , with a sensitivity of 62 % overall , 81 % in untreated patients and only 20 % in treated patients .
	manualset3
146488	8	409496	5	NULL	NULL	0	NULL	81 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection of DNA by PCR was the most useful test especially in untreated patients , with a sensitivity of 62 % overall , 81 % in untreated patients and only 20 % in treated patients .
	manualset3
146489	9	409496	5	NULL	NULL	0	NULL	untreated patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection of DNA by PCR was the most useful test especially in untreated patients , with a sensitivity of 62 % overall , 81 % in untreated patients and only 20 % in treated patients .
	manualset3
146490	10	409496	5	NULL	NULL	0	NULL	20 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection of DNA by PCR was the most useful test especially in untreated patients , with a sensitivity of 62 % overall , 81 % in untreated patients and only 20 % in treated patients .
	manualset3
146491	11	409496	5	NULL	NULL	0	NULL	treated patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection of DNA by PCR was the most useful test especially in untreated patients , with a sensitivity of 62 % overall , 81 % in untreated patients and only 20 % in treated patients .
	manualset3
146492	1	409497	5	NULL	NULL	0	NULL	detection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection of H5 HA protein demonstrates the logical extension of using these nanoparticle mimics as a safe positive control in the detection of influenza , making this a vital step in improving influenza detection methodology .
	manualset3
146493	2	409497	5	NULL	NULL	0	NULL	H5 HA protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection of H5 HA protein demonstrates the logical extension of using these nanoparticle mimics as a safe positive control in the detection of influenza , making this a vital step in improving influenza detection methodology .
	manualset3
146494	3	409497	5	NULL	NULL	0	NULL	logical extension	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection of H5 HA protein demonstrates the logical extension of using these nanoparticle mimics as a safe positive control in the detection of influenza , making this a vital step in improving influenza detection methodology .
	manualset3
146495	4	409497	5	NULL	NULL	0	NULL	nanoparticle mimics 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection of H5 HA protein demonstrates the logical extension of using these nanoparticle mimics as a safe positive control in the detection of influenza , making this a vital step in improving influenza detection methodology .
	manualset3
146496	5	409497	5	NULL	NULL	0	NULL	safe positive control	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection of H5 HA protein demonstrates the logical extension of using these nanoparticle mimics as a safe positive control in the detection of influenza , making this a vital step in improving influenza detection methodology .
	manualset3
146497	6	409497	5	NULL	NULL	0	NULL	detection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection of H5 HA protein demonstrates the logical extension of using these nanoparticle mimics as a safe positive control in the detection of influenza , making this a vital step in improving influenza detection methodology .
	manualset3
146498	7	409497	5	NULL	NULL	0	NULL	influenza 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection of H5 HA protein demonstrates the logical extension of using these nanoparticle mimics as a safe positive control in the detection of influenza , making this a vital step in improving influenza detection methodology .
	manualset3
146499	8	409497	5	NULL	NULL	0	NULL	vital step	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection of H5 HA protein demonstrates the logical extension of using these nanoparticle mimics as a safe positive control in the detection of influenza , making this a vital step in improving influenza detection methodology .
	manualset3
146500	9	409497	5	NULL	NULL	0	NULL	influenza detection methodology 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection of H5 HA protein demonstrates the logical extension of using these nanoparticle mimics as a safe positive control in the detection of influenza , making this a vital step in improving influenza detection methodology .
	manualset3
146501	1	409498	5	NULL	NULL	0	NULL	detection thresholds	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection thresholds for non-painful stimuli ( warmth , cold and electrical stimuli ) seemed to be less affected in the fibromyalgia patients , with only the detection threshold for cold being lower at both sites .
	manualset3
146502	2	409498	5	NULL	NULL	0	NULL	non-painful stimuli	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection thresholds for non-painful stimuli ( warmth , cold and electrical stimuli ) seemed to be less affected in the fibromyalgia patients , with only the detection threshold for cold being lower at both sites .
	manualset3
146503	3	409498	5	NULL	NULL	0	NULL	warmth 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection thresholds for non-painful stimuli ( warmth , cold and electrical stimuli ) seemed to be less affected in the fibromyalgia patients , with only the detection threshold for cold being lower at both sites .
	manualset3
146504	4	409498	5	NULL	NULL	0	NULL	cold 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection thresholds for non-painful stimuli ( warmth , cold and electrical stimuli ) seemed to be less affected in the fibromyalgia patients , with only the detection threshold for cold being lower at both sites .
	manualset3
146505	5	409498	5	NULL	NULL	0	NULL	electrical stimuli	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection thresholds for non-painful stimuli ( warmth , cold and electrical stimuli ) seemed to be less affected in the fibromyalgia patients , with only the detection threshold for cold being lower at both sites .
	manualset3
146506	6	409498	5	NULL	NULL	0	NULL	fibromyalgia patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection thresholds for non-painful stimuli ( warmth , cold and electrical stimuli ) seemed to be less affected in the fibromyalgia patients , with only the detection threshold for cold being lower at both sites .
	manualset3
146507	7	409498	5	NULL	NULL	0	NULL	detection threshold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection thresholds for non-painful stimuli ( warmth , cold and electrical stimuli ) seemed to be less affected in the fibromyalgia patients , with only the detection threshold for cold being lower at both sites .
	manualset3
146508	8	409498	5	NULL	NULL	0	NULL	cold 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection thresholds for non-painful stimuli ( warmth , cold and electrical stimuli ) seemed to be less affected in the fibromyalgia patients , with only the detection threshold for cold being lower at both sites .
	manualset3
148674	9	409498	5	NULL	NULL	0	NULL	sites	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The detection thresholds for non-painful stimuli ( warmth , cold and electrical stimuli ) seemed to be less affected in the fibromyalgia patients , with only the detection threshold for cold being lower at both sites .
	manualset3
146509	1	409499	5	NULL	NULL	0	NULL	determination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of cord blood insulin offers the opportunity of direct diagnostics on the child in contrast to maternal ppoGTT .
	manualset3
146510	2	409499	5	NULL	NULL	0	NULL	cord blood insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of cord blood insulin offers the opportunity of direct diagnostics on the child in contrast to maternal ppoGTT .
	manualset3
146511	3	409499	5	NULL	NULL	0	NULL	opportunity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of cord blood insulin offers the opportunity of direct diagnostics on the child in contrast to maternal ppoGTT .
	manualset3
146512	4	409499	5	NULL	NULL	0	NULL	direct diagnostics 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of cord blood insulin offers the opportunity of direct diagnostics on the child in contrast to maternal ppoGTT .
	manualset3
146513	5	409499	5	NULL	NULL	0	NULL	child 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of cord blood insulin offers the opportunity of direct diagnostics on the child in contrast to maternal ppoGTT .
	manualset3
146514	6	409499	5	NULL	NULL	0	NULL	maternal ppoGTT	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of cord blood insulin offers the opportunity of direct diagnostics on the child in contrast to maternal ppoGTT .
	manualset3
146515	1	409500	5	NULL	NULL	0	NULL	determination 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of the N-terminal groups and the order of splitting allowed the location of the fragments in the polypeptide chain : P3 ( a -- c ) , P2 ( d -- g ) , P4 ( h ) ; T1A ( a -- c ) , T3 ( d ) , T1C ( e -- f ) , T2 ( g ) , T1B ( h ) .
	manualset3
146516	2	409500	5	NULL	NULL	0	NULL	N-terminal groups	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of the N-terminal groups and the order of splitting allowed the location of the fragments in the polypeptide chain : P3 ( a -- c ) , P2 ( d -- g ) , P4 ( h ) ; T1A ( a -- c ) , T3 ( d ) , T1C ( e -- f ) , T2 ( g ) , T1B ( h ) .
	manualset3
146517	3	409500	5	NULL	NULL	0	NULL	location 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of the N-terminal groups and the order of splitting allowed the location of the fragments in the polypeptide chain : P3 ( a -- c ) , P2 ( d -- g ) , P4 ( h ) ; T1A ( a -- c ) , T3 ( d ) , T1C ( e -- f ) , T2 ( g ) , T1B ( h ) .
	manualset3
146518	4	409500	5	NULL	NULL	0	NULL	fragments 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of the N-terminal groups and the order of splitting allowed the location of the fragments in the polypeptide chain : P3 ( a -- c ) , P2 ( d -- g ) , P4 ( h ) ; T1A ( a -- c ) , T3 ( d ) , T1C ( e -- f ) , T2 ( g ) , T1B ( h ) .
	manualset3
146519	5	409500	5	NULL	NULL	0	NULL	polypeptide chain	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of the N-terminal groups and the order of splitting allowed the location of the fragments in the polypeptide chain : P3 ( a -- c ) , P2 ( d -- g ) , P4 ( h ) ; T1A ( a -- c ) , T3 ( d ) , T1C ( e -- f ) , T2 ( g ) , T1B ( h ) .
	manualset3
146520	6	409500	5	NULL	NULL	0	NULL	P3 ( a -- c ) 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of the N-terminal groups and the order of splitting allowed the location of the fragments in the polypeptide chain : P3 ( a -- c ) , P2 ( d -- g ) , P4 ( h ) ; T1A ( a -- c ) , T3 ( d ) , T1C ( e -- f ) , T2 ( g ) , T1B ( h ) .
	manualset3
146521	7	409500	5	NULL	NULL	0	NULL	P2 ( d -- g )	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of the N-terminal groups and the order of splitting allowed the location of the fragments in the polypeptide chain : P3 ( a -- c ) , P2 ( d -- g ) , P4 ( h ) ; T1A ( a -- c ) , T3 ( d ) , T1C ( e -- f ) , T2 ( g ) , T1B ( h ) .
	manualset3
146522	8	409500	5	NULL	NULL	0	NULL	P4 ( h )	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of the N-terminal groups and the order of splitting allowed the location of the fragments in the polypeptide chain : P3 ( a -- c ) , P2 ( d -- g ) , P4 ( h ) ; T1A ( a -- c ) , T3 ( d ) , T1C ( e -- f ) , T2 ( g ) , T1B ( h ) .
	manualset3
146523	9	409500	5	NULL	NULL	0	NULL	T1A ( a -- c )	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of the N-terminal groups and the order of splitting allowed the location of the fragments in the polypeptide chain : P3 ( a -- c ) , P2 ( d -- g ) , P4 ( h ) ; T1A ( a -- c ) , T3 ( d ) , T1C ( e -- f ) , T2 ( g ) , T1B ( h ) .
	manualset3
146524	10	409500	5	NULL	NULL	0	NULL	T3 ( d ) 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of the N-terminal groups and the order of splitting allowed the location of the fragments in the polypeptide chain : P3 ( a -- c ) , P2 ( d -- g ) , P4 ( h ) ; T1A ( a -- c ) , T3 ( d ) , T1C ( e -- f ) , T2 ( g ) , T1B ( h ) .
	manualset3
146525	11	409500	5	NULL	NULL	0	NULL	T1C ( e -- f ) 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of the N-terminal groups and the order of splitting allowed the location of the fragments in the polypeptide chain : P3 ( a -- c ) , P2 ( d -- g ) , P4 ( h ) ; T1A ( a -- c ) , T3 ( d ) , T1C ( e -- f ) , T2 ( g ) , T1B ( h ) .
	manualset3
146526	12	409500	5	NULL	NULL	0	NULL	T2 ( g ) 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of the N-terminal groups and the order of splitting allowed the location of the fragments in the polypeptide chain : P3 ( a -- c ) , P2 ( d -- g ) , P4 ( h ) ; T1A ( a -- c ) , T3 ( d ) , T1C ( e -- f ) , T2 ( g ) , T1B ( h ) .
	manualset3
146527	13	409500	5	NULL	NULL	0	NULL	T1B ( h )	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of the N-terminal groups and the order of splitting allowed the location of the fragments in the polypeptide chain : P3 ( a -- c ) , P2 ( d -- g ) , P4 ( h ) ; T1A ( a -- c ) , T3 ( d ) , T1C ( e -- f ) , T2 ( g ) , T1B ( h ) .
	manualset3
146528	1	409501	5	NULL	NULL	0	NULL	simple technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple technique for the measurement of plasma heparin concentration during anticoagulant therapy .
	manualset3
146529	2	409501	5	NULL	NULL	0	NULL	measurement 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple technique for the measurement of plasma heparin concentration during anticoagulant therapy .
	manualset3
146530	3	409501	5	NULL	NULL	0	NULL	plasma heparin concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple technique for the measurement of plasma heparin concentration during anticoagulant therapy .
	manualset3
146531	4	409501	5	NULL	NULL	0	NULL	anticoagulant therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple technique for the measurement of plasma heparin concentration during anticoagulant therapy .
	manualset3
146532	1	409502	5	NULL	NULL	0	NULL	determination 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of the concentration of lead in the blood shows that this factor increases among treated subjects in a constant way , independently of the dose and the duration of the treatment .
	manualset3
146533	2	409502	5	NULL	NULL	0	NULL	concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of the concentration of lead in the blood shows that this factor increases among treated subjects in a constant way , independently of the dose and the duration of the treatment .
	manualset3
146534	3	409502	5	NULL	NULL	0	NULL	lead 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of the concentration of lead in the blood shows that this factor increases among treated subjects in a constant way , independently of the dose and the duration of the treatment .
	manualset3
146535	4	409502	5	NULL	NULL	0	NULL	blood 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of the concentration of lead in the blood shows that this factor increases among treated subjects in a constant way , independently of the dose and the duration of the treatment .
	manualset3
146536	5	409502	5	NULL	NULL	0	NULL	factor 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of the concentration of lead in the blood shows that this factor increases among treated subjects in a constant way , independently of the dose and the duration of the treatment .
	manualset3
146537	6	409502	5	NULL	NULL	0	NULL	treated subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of the concentration of lead in the blood shows that this factor increases among treated subjects in a constant way , independently of the dose and the duration of the treatment .
	manualset3
146538	7	409502	5	NULL	NULL	0	NULL	dose 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of the concentration of lead in the blood shows that this factor increases among treated subjects in a constant way , independently of the dose and the duration of the treatment .
	manualset3
146539	8	409502	5	NULL	NULL	0	NULL	duration 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of the concentration of lead in the blood shows that this factor increases among treated subjects in a constant way , independently of the dose and the duration of the treatment .
	manualset3
146540	9	409502	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of the concentration of lead in the blood shows that this factor increases among treated subjects in a constant way , independently of the dose and the duration of the treatment .
	manualset3
146541	1	409503	5	NULL	NULL	0	NULL	deuterium isotope effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The deuterium isotope effect was measured using ( 1-R ) - ( 1-14C , 1 -2 H ) ethanol .
	manualset3
146542	2	409503	5	NULL	NULL	0	NULL	( 1-R ) - ( 1-14C , 1 -2 H ) ethanol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The deuterium isotope effect was measured using ( 1-R ) - ( 1-14C , 1 -2 H ) ethanol .
	manualset3
146543	1	409504	5	NULL	NULL	0	NULL	developed method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The developed method is applicable to a broad substrate scope and has significant potential for the synthesis of unnatural amino acids with a triazole side chain .
	manualset3
146544	2	409504	5	NULL	NULL	0	NULL	broad substrate scope	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The developed method is applicable to a broad substrate scope and has significant potential for the synthesis of unnatural amino acids with a triazole side chain .
	manualset3
146545	3	409504	5	NULL	NULL	0	NULL	significant potential	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The developed method is applicable to a broad substrate scope and has significant potential for the synthesis of unnatural amino acids with a triazole side chain .
	manualset3
146546	4	409504	5	NULL	NULL	0	NULL	synthesis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The developed method is applicable to a broad substrate scope and has significant potential for the synthesis of unnatural amino acids with a triazole side chain .
	manualset3
146547	5	409504	5	NULL	NULL	0	NULL	unnatural amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The developed method is applicable to a broad substrate scope and has significant potential for the synthesis of unnatural amino acids with a triazole side chain .
	manualset3
146548	6	409504	5	NULL	NULL	0	NULL	triazole side chain	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The developed method is applicable to a broad substrate scope and has significant potential for the synthesis of unnatural amino acids with a triazole side chain .
	manualset3
146549	1	409505	5	NULL	NULL	0	NULL	developing model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The developing model for ligand-accessible space within the estrogen receptor suggests that Z-phenylvinyl estradiols may provide interesting and useful probes for mapping the receptor .
	manualset3
146550	2	409505	5	NULL	NULL	0	NULL	ligand-accessible space	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The developing model for ligand-accessible space within the estrogen receptor suggests that Z-phenylvinyl estradiols may provide interesting and useful probes for mapping the receptor .
	manualset3
146551	3	409505	5	NULL	NULL	0	NULL	estrogen receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The developing model for ligand-accessible space within the estrogen receptor suggests that Z-phenylvinyl estradiols may provide interesting and useful probes for mapping the receptor .
	manualset3
146552	4	409505	5	NULL	NULL	0	NULL	Z-phenylvinyl estradiols 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The developing model for ligand-accessible space within the estrogen receptor suggests that Z-phenylvinyl estradiols may provide interesting and useful probes for mapping the receptor .
	manualset3
146553	5	409505	5	NULL	NULL	0	NULL	probes 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The developing model for ligand-accessible space within the estrogen receptor suggests that Z-phenylvinyl estradiols may provide interesting and useful probes for mapping the receptor .
	manualset3
146554	6	409505	5	NULL	NULL	0	NULL	receptor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The developing model for ligand-accessible space within the estrogen receptor suggests that Z-phenylvinyl estradiols may provide interesting and useful probes for mapping the receptor .
	manualset3
146555	1	409506	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of `` selective '' drugs targeting oxytocin/vasopressin receptors has enormously progressed since the original synthesis of oxytocin more than 50 years ago .
	manualset3
146556	2	409506	5	NULL	NULL	0	NULL	`` selective '' drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of `` selective '' drugs targeting oxytocin/vasopressin receptors has enormously progressed since the original synthesis of oxytocin more than 50 years ago .
	manualset3
146557	3	409506	5	NULL	NULL	0	NULL	oxytocin/vasopressin receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of `` selective '' drugs targeting oxytocin/vasopressin receptors has enormously progressed since the original synthesis of oxytocin more than 50 years ago .
	manualset3
146558	4	409506	5	NULL	NULL	0	NULL	 original synthesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of `` selective '' drugs targeting oxytocin/vasopressin receptors has enormously progressed since the original synthesis of oxytocin more than 50 years ago .
	manualset3
146559	5	409506	5	NULL	NULL	0	NULL	oxytocin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of `` selective '' drugs targeting oxytocin/vasopressin receptors has enormously progressed since the original synthesis of oxytocin more than 50 years ago .
	manualset3
146560	6	409506	5	NULL	NULL	0	NULL	50 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of `` selective '' drugs targeting oxytocin/vasopressin receptors has enormously progressed since the original synthesis of oxytocin more than 50 years ago .
	manualset3
146561	1	409507	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of additional prosthetic and biologic solutions may require a change in the way glenoid bone loss and component fixation are conceptualized .
	manualset3
146562	2	409507	5	NULL	NULL	0	NULL	prosthetic and biologic solutions	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of additional prosthetic and biologic solutions may require a change in the way glenoid bone loss and component fixation are conceptualized .
	manualset3
146563	3	409507	5	NULL	NULL	0	NULL	change 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of additional prosthetic and biologic solutions may require a change in the way glenoid bone loss and component fixation are conceptualized .
	manualset3
146564	4	409507	5	NULL	NULL	0	NULL	glenoid bone loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of additional prosthetic and biologic solutions may require a change in the way glenoid bone loss and component fixation are conceptualized .
	manualset3
146565	5	409507	5	NULL	NULL	0	NULL	component fixation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of additional prosthetic and biologic solutions may require a change in the way glenoid bone loss and component fixation are conceptualized .
	manualset3
146566	1	409508	5	NULL	NULL	0	NULL	Chronic nonspecific pneumonia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Chronic nonspecific pneumonia in patients with tubercular changes of the lungs ) .
	manualset3
146567	2	409508	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Chronic nonspecific pneumonia in patients with tubercular changes of the lungs ) .
	manualset3
146568	3	409508	5	NULL	NULL	0	NULL	tubercular changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Chronic nonspecific pneumonia in patients with tubercular changes of the lungs ) .
	manualset3
146569	4	409508	5	NULL	NULL	0	NULL	lungs 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Chronic nonspecific pneumonia in patients with tubercular changes of the lungs ) .
	manualset3
146570	1	409509	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of apheresis technologies brought significant benefits to the patient including improving the access to specialty products such as HLA-matched platelets .
	manualset3
146571	2	409509	5	NULL	NULL	0	NULL	apheresis technologies	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of apheresis technologies brought significant benefits to the patient including improving the access to specialty products such as HLA-matched platelets .
	manualset3
146572	3	409509	5	NULL	NULL	0	NULL	benefits 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of apheresis technologies brought significant benefits to the patient including improving the access to specialty products such as HLA-matched platelets .
	manualset3
146573	4	409509	5	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of apheresis technologies brought significant benefits to the patient including improving the access to specialty products such as HLA-matched platelets .
	manualset3
146574	5	409509	5	NULL	NULL	0	NULL	access 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of apheresis technologies brought significant benefits to the patient including improving the access to specialty products such as HLA-matched platelets .
	manualset3
146575	6	409509	5	NULL	NULL	0	NULL	specialty products	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of apheresis technologies brought significant benefits to the patient including improving the access to specialty products such as HLA-matched platelets .
	manualset3
146576	7	409509	5	NULL	NULL	0	NULL	HLA-matched platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of apheresis technologies brought significant benefits to the patient including improving the access to specialty products such as HLA-matched platelets .
	manualset3
146577	1	409510	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of classification schemes for RA in the last 40 years has followed the increasingly precise understanding of the nature of the clinical disease and the recognition of the different requirements of classification methods in clinic and population settings .
	manualset3
146578	2	409510	5	NULL	NULL	0	NULL	classification schemes	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of classification schemes for RA in the last 40 years has followed the increasingly precise understanding of the nature of the clinical disease and the recognition of the different requirements of classification methods in clinic and population settings .
	manualset3
146579	3	409510	5	NULL	NULL	0	NULL	RA 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of classification schemes for RA in the last 40 years has followed the increasingly precise understanding of the nature of the clinical disease and the recognition of the different requirements of classification methods in clinic and population settings .
	manualset3
146580	4	409510	5	NULL	NULL	0	NULL	last 40 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of classification schemes for RA in the last 40 years has followed the increasingly precise understanding of the nature of the clinical disease and the recognition of the different requirements of classification methods in clinic and population settings .
	manualset3
146581	5	409510	5	NULL	NULL	0	NULL	understanding 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of classification schemes for RA in the last 40 years has followed the increasingly precise understanding of the nature of the clinical disease and the recognition of the different requirements of classification methods in clinic and population settings .
	manualset3
146582	6	409510	5	NULL	NULL	0	NULL	nature 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of classification schemes for RA in the last 40 years has followed the increasingly precise understanding of the nature of the clinical disease and the recognition of the different requirements of classification methods in clinic and population settings .
	manualset3
146583	7	409510	5	NULL	NULL	0	NULL	clinical disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of classification schemes for RA in the last 40 years has followed the increasingly precise understanding of the nature of the clinical disease and the recognition of the different requirements of classification methods in clinic and population settings .
	manualset3
146584	8	409510	5	NULL	NULL	0	NULL	recognition 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of classification schemes for RA in the last 40 years has followed the increasingly precise understanding of the nature of the clinical disease and the recognition of the different requirements of classification methods in clinic and population settings .
	manualset3
146585	9	409510	5	NULL	NULL	0	NULL	requirements 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of classification schemes for RA in the last 40 years has followed the increasingly precise understanding of the nature of the clinical disease and the recognition of the different requirements of classification methods in clinic and population settings .
	manualset3
146586	10	409510	5	NULL	NULL	0	NULL	classification methods 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of classification schemes for RA in the last 40 years has followed the increasingly precise understanding of the nature of the clinical disease and the recognition of the different requirements of classification methods in clinic and population settings .
	manualset3
146587	11	409510	5	NULL	NULL	0	NULL	clinic 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of classification schemes for RA in the last 40 years has followed the increasingly precise understanding of the nature of the clinical disease and the recognition of the different requirements of classification methods in clinic and population settings .
	manualset3
146588	12	409510	5	NULL	NULL	0	NULL	population settings	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of classification schemes for RA in the last 40 years has followed the increasingly precise understanding of the nature of the clinical disease and the recognition of the different requirements of classification methods in clinic and population settings .
	manualset3
146589	1	409511	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of glomerulosclerosis was studied in murine chronic graft-versus-host disease ( GvHD ) , which is a model for human systemic lupus erythematosus .
	manualset3
146590	2	409511	5	NULL	NULL	0	NULL	glomerulosclerosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of glomerulosclerosis was studied in murine chronic graft-versus-host disease ( GvHD ) , which is a model for human systemic lupus erythematosus .
	manualset3
146591	3	409511	5	NULL	NULL	0	NULL	murine chronic graft-versus-host disease ( GvHD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of glomerulosclerosis was studied in murine chronic graft-versus-host disease ( GvHD ) , which is a model for human systemic lupus erythematosus .
	manualset3
146592	4	409511	5	NULL	NULL	0	NULL	model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of glomerulosclerosis was studied in murine chronic graft-versus-host disease ( GvHD ) , which is a model for human systemic lupus erythematosus .
	manualset3
146593	5	409511	5	NULL	NULL	0	NULL	human systemic lupus erythematosus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of glomerulosclerosis was studied in murine chronic graft-versus-host disease ( GvHD ) , which is a model for human systemic lupus erythematosus .
	manualset3
146594	1	409512	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of inhibitory antibodies to factor VIII ( FVIII ) occurs in approximately 30 % to 40 % of patients with severe hemophilia A. Management options for patients with inhibitor include eradicating it via immune tolerance induction ( ITI ) or treating bleeding episodes with large quantities of hemostatic agents .
	manualset3
146595	2	409512	5	NULL	NULL	NULL	NULL	inhibitory antibodies to factor VIII ( FVIII ) 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The development of inhibitory antibodies to factor VIII ( FVIII ) occurs in approximately 30 % to 40 % of patients with severe hemophilia A. Management options for patients with inhibitor include eradicating it via immune tolerance induction ( ITI ) or treating bleeding episodes with large quantities of hemostatic agents .
	manualset3
146596	3	409512	5	NULL	NULL	0	NULL	30 % to 40 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of inhibitory antibodies to factor VIII ( FVIII ) occurs in approximately 30 % to 40 % of patients with severe hemophilia A. Management options for patients with inhibitor include eradicating it via immune tolerance induction ( ITI ) or treating bleeding episodes with large quantities of hemostatic agents .
	manualset3
146597	4	409512	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of inhibitory antibodies to factor VIII ( FVIII ) occurs in approximately 30 % to 40 % of patients with severe hemophilia A. Management options for patients with inhibitor include eradicating it via immune tolerance induction ( ITI ) or treating bleeding episodes with large quantities of hemostatic agents .
	manualset3
146598	5	409512	5	NULL	NULL	0	NULL	severe hemophilia A	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of inhibitory antibodies to factor VIII ( FVIII ) occurs in approximately 30 % to 40 % of patients with severe hemophilia A. Management options for patients with inhibitor include eradicating it via immune tolerance induction ( ITI ) or treating bleeding episodes with large quantities of hemostatic agents .
	manualset3
146599	6	409512	5	NULL	NULL	0	NULL	Management options	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of inhibitory antibodies to factor VIII ( FVIII ) occurs in approximately 30 % to 40 % of patients with severe hemophilia A. Management options for patients with inhibitor include eradicating it via immune tolerance induction ( ITI ) or treating bleeding episodes with large quantities of hemostatic agents .
	manualset3
146600	7	409512	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of inhibitory antibodies to factor VIII ( FVIII ) occurs in approximately 30 % to 40 % of patients with severe hemophilia A. Management options for patients with inhibitor include eradicating it via immune tolerance induction ( ITI ) or treating bleeding episodes with large quantities of hemostatic agents .
	manualset3
146601	8	409512	5	NULL	NULL	0	NULL	inhibitor 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of inhibitory antibodies to factor VIII ( FVIII ) occurs in approximately 30 % to 40 % of patients with severe hemophilia A. Management options for patients with inhibitor include eradicating it via immune tolerance induction ( ITI ) or treating bleeding episodes with large quantities of hemostatic agents .
	manualset3
146602	9	409512	5	NULL	NULL	0	NULL	immune tolerance induction ( ITI ) 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of inhibitory antibodies to factor VIII ( FVIII ) occurs in approximately 30 % to 40 % of patients with severe hemophilia A. Management options for patients with inhibitor include eradicating it via immune tolerance induction ( ITI ) or treating bleeding episodes with large quantities of hemostatic agents .
	manualset3
146603	10	409512	5	NULL	NULL	0	NULL	bleeding episodes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of inhibitory antibodies to factor VIII ( FVIII ) occurs in approximately 30 % to 40 % of patients with severe hemophilia A. Management options for patients with inhibitor include eradicating it via immune tolerance induction ( ITI ) or treating bleeding episodes with large quantities of hemostatic agents .
	manualset3
146604	11	409512	5	NULL	NULL	0	NULL	large quantities	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of inhibitory antibodies to factor VIII ( FVIII ) occurs in approximately 30 % to 40 % of patients with severe hemophilia A. Management options for patients with inhibitor include eradicating it via immune tolerance induction ( ITI ) or treating bleeding episodes with large quantities of hemostatic agents .
	manualset3
146605	12	409512	5	NULL	NULL	0	NULL	hemostatic agents	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of inhibitory antibodies to factor VIII ( FVIII ) occurs in approximately 30 % to 40 % of patients with severe hemophilia A. Management options for patients with inhibitor include eradicating it via immune tolerance induction ( ITI ) or treating bleeding episodes with large quantities of hemostatic agents .
	manualset3
146606	1	409513	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of lasers for medical use , which became known as low-level laser therapy ( LLLT ) or photobiomodulation , followed in 1967 .
	manualset3
146607	2	409513	5	NULL	NULL	0	NULL	lasers 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of lasers for medical use , which became known as low-level laser therapy ( LLLT ) or photobiomodulation , followed in 1967 .
	manualset3
146608	3	409513	5	NULL	NULL	0	NULL	medical use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of lasers for medical use , which became known as low-level laser therapy ( LLLT ) or photobiomodulation , followed in 1967 .
	manualset3
146609	4	409513	5	NULL	NULL	0	NULL	low-level laser therapy ( LLLT ) or photobiomodulation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of lasers for medical use , which became known as low-level laser therapy ( LLLT ) or photobiomodulation , followed in 1967 .
	manualset3
146610	5	409513	5	NULL	NULL	0	NULL	1967 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of lasers for medical use , which became known as low-level laser therapy ( LLLT ) or photobiomodulation , followed in 1967 .
	manualset3
146611	1	409514	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of molecular methods to typify HLA alleles and recent updates of their nomenclature has contributed to a better understanding of this system .
	manualset3
146612	2	409514	5	NULL	NULL	0	NULL	molecular methods 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of molecular methods to typify HLA alleles and recent updates of their nomenclature has contributed to a better understanding of this system .
	manualset3
146613	3	409514	5	NULL	NULL	0	NULL	HLA alleles	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of molecular methods to typify HLA alleles and recent updates of their nomenclature has contributed to a better understanding of this system .
	manualset3
146614	4	409514	5	NULL	NULL	0	NULL	updates 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of molecular methods to typify HLA alleles and recent updates of their nomenclature has contributed to a better understanding of this system .
	manualset3
146615	5	409514	5	NULL	NULL	0	NULL	nomenclature 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of molecular methods to typify HLA alleles and recent updates of their nomenclature has contributed to a better understanding of this system .
	manualset3
146616	6	409514	5	NULL	NULL	0	NULL	system 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of molecular methods to typify HLA alleles and recent updates of their nomenclature has contributed to a better understanding of this system .
	manualset3
146617	1	409515	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of porcine models of obesity and the metabolic syndrome .
	manualset3
146618	2	409515	5	NULL	NULL	0	NULL	porcine models 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of porcine models of obesity and the metabolic syndrome .
	manualset3
146619	3	409515	5	NULL	NULL	0	NULL	obesity 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of porcine models of obesity and the metabolic syndrome .
	manualset3
146620	4	409515	5	NULL	NULL	0	NULL	metabolic syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of porcine models of obesity and the metabolic syndrome .
	manualset3
146621	1	409516	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of reliable and reproducible small and large animal models is essential for the study of the unique immunological and biological aspects of vascularized composite allografts and to translate such novel immunoregulatory and tolerance-inducing strategies and therapeutic concepts from the bench to bedside .
	manualset3
146622	2	409516	5	NULL	NULL	0	NULL	animal models	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of reliable and reproducible small and large animal models is essential for the study of the unique immunological and biological aspects of vascularized composite allografts and to translate such novel immunoregulatory and tolerance-inducing strategies and therapeutic concepts from the bench to bedside .
	manualset3
146623	3	409516	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of reliable and reproducible small and large animal models is essential for the study of the unique immunological and biological aspects of vascularized composite allografts and to translate such novel immunoregulatory and tolerance-inducing strategies and therapeutic concepts from the bench to bedside .
	manualset3
146624	4	409516	5	NULL	NULL	0	NULL	immunological aspects	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of reliable and reproducible small and large animal models is essential for the study of the unique immunological and biological aspects of vascularized composite allografts and to translate such novel immunoregulatory and tolerance-inducing strategies and therapeutic concepts from the bench to bedside .
	manualset3
146625	5	409516	5	NULL	NULL	0	NULL	biological aspects 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of reliable and reproducible small and large animal models is essential for the study of the unique immunological and biological aspects of vascularized composite allografts and to translate such novel immunoregulatory and tolerance-inducing strategies and therapeutic concepts from the bench to bedside .
	manualset3
146626	6	409516	5	NULL	NULL	0	NULL	vascularized composite allografts 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of reliable and reproducible small and large animal models is essential for the study of the unique immunological and biological aspects of vascularized composite allografts and to translate such novel immunoregulatory and tolerance-inducing strategies and therapeutic concepts from the bench to bedside .
	manualset3
146627	7	409516	5	NULL	NULL	0	NULL	immunoregulatory strategies 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of reliable and reproducible small and large animal models is essential for the study of the unique immunological and biological aspects of vascularized composite allografts and to translate such novel immunoregulatory and tolerance-inducing strategies and therapeutic concepts from the bench to bedside .
	manualset3
146628	8	409516	5	NULL	NULL	0	NULL	tolerance-inducing strategies 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of reliable and reproducible small and large animal models is essential for the study of the unique immunological and biological aspects of vascularized composite allografts and to translate such novel immunoregulatory and tolerance-inducing strategies and therapeutic concepts from the bench to bedside .
	manualset3
146629	9	409516	5	NULL	NULL	0	NULL	therapeutic concepts	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of reliable and reproducible small and large animal models is essential for the study of the unique immunological and biological aspects of vascularized composite allografts and to translate such novel immunoregulatory and tolerance-inducing strategies and therapeutic concepts from the bench to bedside .
	manualset3
146630	1	409517	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of symptoms was noted as was the clinical state on admission and after treatment .
	manualset3
146631	2	409517	5	NULL	NULL	0	NULL	symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of symptoms was noted as was the clinical state on admission and after treatment .
	manualset3
146632	3	409517	5	NULL	NULL	0	NULL	clinical state	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of symptoms was noted as was the clinical state on admission and after treatment .
	manualset3
146633	4	409517	5	NULL	NULL	0	NULL	admission 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of symptoms was noted as was the clinical state on admission and after treatment .
	manualset3
146634	5	409517	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of symptoms was noted as was the clinical state on admission and after treatment .
	manualset3
146635	1	409518	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of the MC3T3-E1 cells can be divided into three major stages , namely , proliferation , differentiation , and mineralization .
	manualset3
146636	2	409518	5	NULL	NULL	0	NULL	MC3T3-E1 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of the MC3T3-E1 cells can be divided into three major stages , namely , proliferation , differentiation , and mineralization .
	manualset3
146637	3	409518	5	NULL	NULL	0	NULL	three major stages	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of the MC3T3-E1 cells can be divided into three major stages , namely , proliferation , differentiation , and mineralization .
	manualset3
146638	4	409518	5	NULL	NULL	0	NULL	proliferation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of the MC3T3-E1 cells can be divided into three major stages , namely , proliferation , differentiation , and mineralization .
	manualset3
146639	5	409518	5	NULL	NULL	0	NULL	differentiation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of the MC3T3-E1 cells can be divided into three major stages , namely , proliferation , differentiation , and mineralization .
	manualset3
146640	6	409518	5	NULL	NULL	0	NULL	mineralization 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of the MC3T3-E1 cells can be divided into three major stages , namely , proliferation , differentiation , and mineralization .
	manualset3
146641	1	409519	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of the Weibel instability during the expansion of a thin plasma foil heated by an intense laser pulse is investigated , using both analytical models and relativistic particle-in-cell simulations .
	manualset3
146642	2	409519	5	NULL	NULL	0	NULL	Weibel instability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of the Weibel instability during the expansion of a thin plasma foil heated by an intense laser pulse is investigated , using both analytical models and relativistic particle-in-cell simulations .
	manualset3
146643	3	409519	5	NULL	NULL	0	NULL	expansion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of the Weibel instability during the expansion of a thin plasma foil heated by an intense laser pulse is investigated , using both analytical models and relativistic particle-in-cell simulations .
	manualset3
146644	4	409519	5	NULL	NULL	0	NULL	thin plasma foil 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of the Weibel instability during the expansion of a thin plasma foil heated by an intense laser pulse is investigated , using both analytical models and relativistic particle-in-cell simulations .
	manualset3
146645	5	409519	5	NULL	NULL	NULL	NULL	intense laser pulse	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The development of the Weibel instability during the expansion of a thin plasma foil heated by an intense laser pulse is investigated , using both analytical models and relativistic particle-in-cell simulations .
	manualset3
146646	6	409519	5	NULL	NULL	0	NULL	analytical models 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of the Weibel instability during the expansion of a thin plasma foil heated by an intense laser pulse is investigated , using both analytical models and relativistic particle-in-cell simulations .
	manualset3
146647	7	409519	5	NULL	NULL	0	NULL	relativistic particle-in-cell simulations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of the Weibel instability during the expansion of a thin plasma foil heated by an intense laser pulse is investigated , using both analytical models and relativistic particle-in-cell simulations .
	manualset3
146648	1	409520	5	NULL	NULL	0	NULL	developmental 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The developmental and phenotypic properties of the hist ( + ) / morph ( - ) foci , hist ( + ) / morph ( + ) foci , and hepatic tumors were compared in rats initiated once neonatally with different doses of diethylnitrosamine and promoted with dietary phenobarbital from weaning .
	manualset3
146649	2	409520	5	NULL	NULL	0	NULL	phenotypic properties 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The developmental and phenotypic properties of the hist ( + ) / morph ( - ) foci , hist ( + ) / morph ( + ) foci , and hepatic tumors were compared in rats initiated once neonatally with different doses of diethylnitrosamine and promoted with dietary phenobarbital from weaning .
	manualset3
146650	3	409520	5	NULL	NULL	0	NULL	hist ( + ) / morph ( - ) foci 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The developmental and phenotypic properties of the hist ( + ) / morph ( - ) foci , hist ( + ) / morph ( + ) foci , and hepatic tumors were compared in rats initiated once neonatally with different doses of diethylnitrosamine and promoted with dietary phenobarbital from weaning .
	manualset3
146651	4	409520	5	NULL	NULL	0	NULL	hist ( + ) / morph ( + ) foci 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The developmental and phenotypic properties of the hist ( + ) / morph ( - ) foci , hist ( + ) / morph ( + ) foci , and hepatic tumors were compared in rats initiated once neonatally with different doses of diethylnitrosamine and promoted with dietary phenobarbital from weaning .
	manualset3
146652	5	409520	5	NULL	NULL	0	NULL	hepatic tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The developmental and phenotypic properties of the hist ( + ) / morph ( - ) foci , hist ( + ) / morph ( + ) foci , and hepatic tumors were compared in rats initiated once neonatally with different doses of diethylnitrosamine and promoted with dietary phenobarbital from weaning .
	manualset3
146653	6	409520	5	NULL	NULL	0	NULL	rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The developmental and phenotypic properties of the hist ( + ) / morph ( - ) foci , hist ( + ) / morph ( + ) foci , and hepatic tumors were compared in rats initiated once neonatally with different doses of diethylnitrosamine and promoted with dietary phenobarbital from weaning .
	manualset3
146654	7	409520	5	NULL	NULL	0	NULL	doses 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The developmental and phenotypic properties of the hist ( + ) / morph ( - ) foci , hist ( + ) / morph ( + ) foci , and hepatic tumors were compared in rats initiated once neonatally with different doses of diethylnitrosamine and promoted with dietary phenobarbital from weaning .
	manualset3
146655	8	409520	5	NULL	NULL	0	NULL	diethylnitrosamine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The developmental and phenotypic properties of the hist ( + ) / morph ( - ) foci , hist ( + ) / morph ( + ) foci , and hepatic tumors were compared in rats initiated once neonatally with different doses of diethylnitrosamine and promoted with dietary phenobarbital from weaning .
	manualset3
146656	9	409520	5	NULL	NULL	0	NULL	dietary phenobarbital	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The developmental and phenotypic properties of the hist ( + ) / morph ( - ) foci , hist ( + ) / morph ( + ) foci , and hepatic tumors were compared in rats initiated once neonatally with different doses of diethylnitrosamine and promoted with dietary phenobarbital from weaning .
	manualset3
146657	10	409520	5	NULL	NULL	0	NULL	weaning 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The developmental and phenotypic properties of the hist ( + ) / morph ( - ) foci , hist ( + ) / morph ( + ) foci , and hepatic tumors were compared in rats initiated once neonatally with different doses of diethylnitrosamine and promoted with dietary phenobarbital from weaning .
	manualset3
146658	1	409521	5	NULL	NULL	0	NULL	developmental status 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The developmental status of muscle fibers was investigated in three cases of myotubular myopathy : one infant with the X-linked recessive form and two adult brothers with the autosomal , probably recessive , form of the disease .
	manualset3
146659	2	409521	5	NULL	NULL	0	NULL	muscle fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The developmental status of muscle fibers was investigated in three cases of myotubular myopathy : one infant with the X-linked recessive form and two adult brothers with the autosomal , probably recessive , form of the disease .
	manualset3
146660	3	409521	5	NULL	NULL	0	NULL	three cases	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The developmental status of muscle fibers was investigated in three cases of myotubular myopathy : one infant with the X-linked recessive form and two adult brothers with the autosomal , probably recessive , form of the disease .
	manualset3
146661	4	409521	5	NULL	NULL	0	NULL	myotubular myopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The developmental status of muscle fibers was investigated in three cases of myotubular myopathy : one infant with the X-linked recessive form and two adult brothers with the autosomal , probably recessive , form of the disease .
	manualset3
146662	5	409521	5	NULL	NULL	0	NULL	one infant 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The developmental status of muscle fibers was investigated in three cases of myotubular myopathy : one infant with the X-linked recessive form and two adult brothers with the autosomal , probably recessive , form of the disease .
	manualset3
146663	6	409521	5	NULL	NULL	0	NULL	X-linked recessive form 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The developmental status of muscle fibers was investigated in three cases of myotubular myopathy : one infant with the X-linked recessive form and two adult brothers with the autosomal , probably recessive , form of the disease .
	manualset3
146664	7	409521	5	NULL	NULL	0	NULL	two adult brothers	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The developmental status of muscle fibers was investigated in three cases of myotubular myopathy : one infant with the X-linked recessive form and two adult brothers with the autosomal , probably recessive , form of the disease .
	manualset3
146665	8	409521	5	NULL	NULL	0	NULL	disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The developmental status of muscle fibers was investigated in three cases of myotubular myopathy : one infant with the X-linked recessive form and two adult brothers with the autosomal , probably recessive , form of the disease .
	manualset3
146666	1	409522	5	NULL	NULL	0	NULL	device 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The device , which is capable of detecting 0.26 milligram of lead per square centimeter of paint ( approximately 3 percent ( by weight ) of lead in a single coat ) beneath ten layers of lead-free paint , has been tested in a preliminary survey of several tenement apartments in New York City .
	manualset3
146667	2	409522	5	NULL	NULL	0	NULL	 0.26 milligram of lead per square centimeter of paint 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The device , which is capable of detecting 0.26 milligram of lead per square centimeter of paint ( approximately 3 percent ( by weight ) of lead in a single coat ) beneath ten layers of lead-free paint , has been tested in a preliminary survey of several tenement apartments in New York City .
	manualset3
146668	3	409522	5	NULL	NULL	0	NULL	3 percent ( by weight )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The device , which is capable of detecting 0.26 milligram of lead per square centimeter of paint ( approximately 3 percent ( by weight ) of lead in a single coat ) beneath ten layers of lead-free paint , has been tested in a preliminary survey of several tenement apartments in New York City .
	manualset3
146669	4	409522	5	NULL	NULL	0	NULL	lead 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The device , which is capable of detecting 0.26 milligram of lead per square centimeter of paint ( approximately 3 percent ( by weight ) of lead in a single coat ) beneath ten layers of lead-free paint , has been tested in a preliminary survey of several tenement apartments in New York City .
	manualset3
146670	5	409522	5	NULL	NULL	0	NULL	single coat	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The device , which is capable of detecting 0.26 milligram of lead per square centimeter of paint ( approximately 3 percent ( by weight ) of lead in a single coat ) beneath ten layers of lead-free paint , has been tested in a preliminary survey of several tenement apartments in New York City .
	manualset3
146671	6	409522	5	NULL	NULL	0	NULL	ten layers	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The device , which is capable of detecting 0.26 milligram of lead per square centimeter of paint ( approximately 3 percent ( by weight ) of lead in a single coat ) beneath ten layers of lead-free paint , has been tested in a preliminary survey of several tenement apartments in New York City .
	manualset3
146672	7	409522	5	NULL	NULL	0	NULL	lead-free paint	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The device , which is capable of detecting 0.26 milligram of lead per square centimeter of paint ( approximately 3 percent ( by weight ) of lead in a single coat ) beneath ten layers of lead-free paint , has been tested in a preliminary survey of several tenement apartments in New York City .
	manualset3
146673	8	409522	5	NULL	NULL	0	NULL	preliminary survey	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The device , which is capable of detecting 0.26 milligram of lead per square centimeter of paint ( approximately 3 percent ( by weight ) of lead in a single coat ) beneath ten layers of lead-free paint , has been tested in a preliminary survey of several tenement apartments in New York City .
	manualset3
146674	9	409522	5	NULL	NULL	0	NULL	tenement apartments	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The device , which is capable of detecting 0.26 milligram of lead per square centimeter of paint ( approximately 3 percent ( by weight ) of lead in a single coat ) beneath ten layers of lead-free paint , has been tested in a preliminary survey of several tenement apartments in New York City .
	manualset3
146675	10	409522	5	NULL	NULL	0	NULL	New York City	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The device , which is capable of detecting 0.26 milligram of lead per square centimeter of paint ( approximately 3 percent ( by weight ) of lead in a single coat ) beneath ten layers of lead-free paint , has been tested in a preliminary survey of several tenement apartments in New York City .
	manualset3
146676	1	409523	5	NULL	NULL	0	NULL	device 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The device achieves focal Electric Capacitive Stimulation ( ECS ) by coupling of single cells and semiconductors , without electrochemical reaction with the substrate .
	manualset3
146677	2	409523	5	NULL	NULL	0	NULL	focal Electric Capacitive Stimulation ( ECS )	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The device achieves focal Electric Capacitive Stimulation ( ECS ) by coupling of single cells and semiconductors , without electrochemical reaction with the substrate .
	manualset3
146678	3	409523	5	NULL	NULL	0	NULL	single cells	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The device achieves focal Electric Capacitive Stimulation ( ECS ) by coupling of single cells and semiconductors , without electrochemical reaction with the substrate .
	manualset3
146679	4	409523	5	NULL	NULL	0	NULL	semiconductors 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The device achieves focal Electric Capacitive Stimulation ( ECS ) by coupling of single cells and semiconductors , without electrochemical reaction with the substrate .
	manualset3
146680	5	409523	5	NULL	NULL	NULL	NULL	electrochemical reaction 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The device achieves focal Electric Capacitive Stimulation ( ECS ) by coupling of single cells and semiconductors , without electrochemical reaction with the substrate .
	manualset3
146681	6	409523	5	NULL	NULL	0	NULL	substrate 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The device achieves focal Electric Capacitive Stimulation ( ECS ) by coupling of single cells and semiconductors , without electrochemical reaction with the substrate .
	manualset3
146682	1	409524	5	NULL	NULL	0	NULL	device 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The device was designed to record breathing movements , nasal and oral flow , position , snore , blood oxygen saturation and heart rate .
	manualset3
146683	2	409524	5	NULL	NULL	0	NULL	breathing movements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The device was designed to record breathing movements , nasal and oral flow , position , snore , blood oxygen saturation and heart rate .
	manualset3
146684	3	409524	5	NULL	NULL	0	NULL	nasal and oral flow	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The device was designed to record breathing movements , nasal and oral flow , position , snore , blood oxygen saturation and heart rate .
	manualset3
146685	4	409524	5	NULL	NULL	0	NULL	position 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The device was designed to record breathing movements , nasal and oral flow , position , snore , blood oxygen saturation and heart rate .
	manualset3
146686	5	409524	5	NULL	NULL	0	NULL	snore 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The device was designed to record breathing movements , nasal and oral flow , position , snore , blood oxygen saturation and heart rate .
	manualset3
146687	6	409524	5	NULL	NULL	0	NULL	blood oxygen saturation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The device was designed to record breathing movements , nasal and oral flow , position , snore , blood oxygen saturation and heart rate .
	manualset3
146688	7	409524	5	NULL	NULL	0	NULL	heart rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The device was designed to record breathing movements , nasal and oral flow , position , snore , blood oxygen saturation and heart rate .
	manualset3
146689	1	409525	5	NULL	NULL	0	NULL	diabetic osteoarthropathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The diabetic osteoarthropathy is an important diabetic complication .
	manualset3
146690	2	409525	5	NULL	NULL	0	NULL	diabetic complication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The diabetic osteoarthropathy is an important diabetic complication .
	manualset3
146691	1	409526	5	NULL	NULL	0	NULL	diabetic state 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The diabetic state of rats induced by one injection of STZ was severely advanced at 10 months after the injection .
	manualset3
146692	2	409526	5	NULL	NULL	0	NULL	rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The diabetic state of rats induced by one injection of STZ was severely advanced at 10 months after the injection .
	manualset3
146693	3	409526	5	NULL	NULL	0	NULL	one injection 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The diabetic state of rats induced by one injection of STZ was severely advanced at 10 months after the injection .
	manualset3
146694	4	409526	5	NULL	NULL	0	NULL	STZ 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The diabetic state of rats induced by one injection of STZ was severely advanced at 10 months after the injection .
	manualset3
146695	5	409526	5	NULL	NULL	0	NULL	10 months	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The diabetic state of rats induced by one injection of STZ was severely advanced at 10 months after the injection .
	manualset3
146696	6	409526	5	NULL	NULL	0	NULL	injection 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diabetic state of rats induced by one injection of STZ was severely advanced at 10 months after the injection .
	manualset3
146697	1	409527	5	NULL	NULL	0	NULL	simulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A simulation of the process was conducted using the bioprocess engineering software SuperPro Designer v6 .0 ( Intelligen , Inc. , Scotch Plains , NJ ) to determine the economic feasibility of the process .
	manualset3
146698	2	409527	5	NULL	NULL	0	NULL	process 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A simulation of the process was conducted using the bioprocess engineering software SuperPro Designer v6 .0 ( Intelligen , Inc. , Scotch Plains , NJ ) to determine the economic feasibility of the process .
	manualset3
146699	3	409527	5	NULL	NULL	0	NULL	bioprocess engineering software SuperPro Designer v6 .0 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A simulation of the process was conducted using the bioprocess engineering software SuperPro Designer v6 .0 ( Intelligen , Inc. , Scotch Plains , NJ ) to determine the economic feasibility of the process .
	manualset3
146700	4	409527	5	NULL	NULL	0	NULL	Intelligen , Inc. 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A simulation of the process was conducted using the bioprocess engineering software SuperPro Designer v6 .0 ( Intelligen , Inc. , Scotch Plains , NJ ) to determine the economic feasibility of the process .
	manualset3
146701	5	409527	5	NULL	NULL	0	NULL	Scotch Plains , NJ 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A simulation of the process was conducted using the bioprocess engineering software SuperPro Designer v6 .0 ( Intelligen , Inc. , Scotch Plains , NJ ) to determine the economic feasibility of the process .
	manualset3
146702	6	409527	5	NULL	NULL	0	NULL	economic feasibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A simulation of the process was conducted using the bioprocess engineering software SuperPro Designer v6 .0 ( Intelligen , Inc. , Scotch Plains , NJ ) to determine the economic feasibility of the process .
	manualset3
146703	7	409527	5	NULL	NULL	0	NULL	process 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A simulation of the process was conducted using the bioprocess engineering software SuperPro Designer v6 .0 ( Intelligen , Inc. , Scotch Plains , NJ ) to determine the economic feasibility of the process .
	manualset3
146704	1	409528	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis , which in all cases was based on radiography , was followed by immediate treatment for shock and surgical intervention whenever possible .
	manualset3
146705	2	409528	5	NULL	NULL	0	NULL	cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis , which in all cases was based on radiography , was followed by immediate treatment for shock and surgical intervention whenever possible .
	manualset3
146706	3	409528	5	NULL	NULL	0	NULL	radiography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis , which in all cases was based on radiography , was followed by immediate treatment for shock and surgical intervention whenever possible .
	manualset3
146707	4	409528	5	NULL	NULL	0	NULL	immediate treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis , which in all cases was based on radiography , was followed by immediate treatment for shock and surgical intervention whenever possible .
	manualset3
146708	5	409528	5	NULL	NULL	0	NULL	shock 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis , which in all cases was based on radiography , was followed by immediate treatment for shock and surgical intervention whenever possible .
	manualset3
146709	6	409528	5	NULL	NULL	0	NULL	surgical intervention 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis , which in all cases was based on radiography , was followed by immediate treatment for shock and surgical intervention whenever possible .
	manualset3
146710	1	409529	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis and management of acid-base imbalance .
	manualset3
146711	2	409529	5	NULL	NULL	0	NULL	management 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis and management of acid-base imbalance .
	manualset3
146712	3	409529	5	NULL	NULL	0	NULL	acid-base imbalance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis and management of acid-base imbalance .
	manualset3
146713	1	409530	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis and treatment of ocular neuroses .
	manualset3
146714	2	409530	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis and treatment of ocular neuroses .
	manualset3
146715	3	409530	5	NULL	NULL	0	NULL	ocular neuroses	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis and treatment of ocular neuroses .
	manualset3
146716	1	409531	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis and treatment of such diseases call for a board of doctors including ophthalmologist , otolaryngologist and oral surgeon .
	manualset3
146717	2	409531	5	NULL	NULL	NULL	NULL	treatment 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The diagnosis and treatment of such diseases call for a board of doctors including ophthalmologist , otolaryngologist and oral surgeon .
	manualset3
146718	3	409531	5	NULL	NULL	0	NULL	diseases 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis and treatment of such diseases call for a board of doctors including ophthalmologist , otolaryngologist and oral surgeon .
	manualset3
146719	4	409531	5	NULL	NULL	0	NULL	board of doctors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis and treatment of such diseases call for a board of doctors including ophthalmologist , otolaryngologist and oral surgeon .
	manualset3
146720	5	409531	5	NULL	NULL	0	NULL	ophthalmologist 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis and treatment of such diseases call for a board of doctors including ophthalmologist , otolaryngologist and oral surgeon .
	manualset3
146721	6	409531	5	NULL	NULL	0	NULL	otolaryngologist 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis and treatment of such diseases call for a board of doctors including ophthalmologist , otolaryngologist and oral surgeon .
	manualset3
146722	7	409531	5	NULL	NULL	0	NULL	oral surgeon	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis and treatment of such diseases call for a board of doctors including ophthalmologist , otolaryngologist and oral surgeon .
	manualset3
146723	1	409532	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis has traditionally rested on measurements of ceruloplasmin and copper in urine and liver , but it remains a challenge due to ambiguous biochemical results that can overlap with healthy carriers .
	manualset3
146724	2	409532	5	NULL	NULL	0	NULL	measurements 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis has traditionally rested on measurements of ceruloplasmin and copper in urine and liver , but it remains a challenge due to ambiguous biochemical results that can overlap with healthy carriers .
	manualset3
146725	3	409532	5	NULL	NULL	0	NULL	ceruloplasmin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis has traditionally rested on measurements of ceruloplasmin and copper in urine and liver , but it remains a challenge due to ambiguous biochemical results that can overlap with healthy carriers .
	manualset3
146726	4	409532	5	NULL	NULL	0	NULL	copper 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis has traditionally rested on measurements of ceruloplasmin and copper in urine and liver , but it remains a challenge due to ambiguous biochemical results that can overlap with healthy carriers .
	manualset3
146727	5	409532	5	NULL	NULL	0	NULL	urine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis has traditionally rested on measurements of ceruloplasmin and copper in urine and liver , but it remains a challenge due to ambiguous biochemical results that can overlap with healthy carriers .
	manualset3
146728	6	409532	5	NULL	NULL	0	NULL	liver 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis has traditionally rested on measurements of ceruloplasmin and copper in urine and liver , but it remains a challenge due to ambiguous biochemical results that can overlap with healthy carriers .
	manualset3
146729	7	409532	5	NULL	NULL	0	NULL	challenge 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis has traditionally rested on measurements of ceruloplasmin and copper in urine and liver , but it remains a challenge due to ambiguous biochemical results that can overlap with healthy carriers .
	manualset3
146730	8	409532	5	NULL	NULL	0	NULL	ambiguous biochemical results	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis has traditionally rested on measurements of ceruloplasmin and copper in urine and liver , but it remains a challenge due to ambiguous biochemical results that can overlap with healthy carriers .
	manualset3
146731	9	409532	5	NULL	NULL	0	NULL	healthy carriers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis has traditionally rested on measurements of ceruloplasmin and copper in urine and liver , but it remains a challenge due to ambiguous biochemical results that can overlap with healthy carriers .
	manualset3
146732	1	409533	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis is confirmed by parasitological examination of the excised nodule .
	manualset3
146733	2	409533	5	NULL	NULL	0	NULL	parasitological examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis is confirmed by parasitological examination of the excised nodule .
	manualset3
146734	3	409533	5	NULL	NULL	0	NULL	excised nodule	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis is confirmed by parasitological examination of the excised nodule .
	manualset3
146735	1	409534	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of FHD continues to require a combination of clinical evaluation and a series of diagnostic tests , often requiring reevaluations over time .
	manualset3
146736	2	409534	5	NULL	NULL	0	NULL	FHD 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of FHD continues to require a combination of clinical evaluation and a series of diagnostic tests , often requiring reevaluations over time .
	manualset3
146737	3	409534	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of FHD continues to require a combination of clinical evaluation and a series of diagnostic tests , often requiring reevaluations over time .
	manualset3
146738	4	409534	5	NULL	NULL	0	NULL	clinical evaluation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of FHD continues to require a combination of clinical evaluation and a series of diagnostic tests , often requiring reevaluations over time .
	manualset3
146739	5	409534	5	NULL	NULL	0	NULL	series 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of FHD continues to require a combination of clinical evaluation and a series of diagnostic tests , often requiring reevaluations over time .
	manualset3
146740	6	409534	5	NULL	NULL	0	NULL	diagnostic tests	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of FHD continues to require a combination of clinical evaluation and a series of diagnostic tests , often requiring reevaluations over time .
	manualset3
146741	7	409534	5	NULL	NULL	0	NULL	reevaluations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of FHD continues to require a combination of clinical evaluation and a series of diagnostic tests , often requiring reevaluations over time .
	manualset3
146742	8	409534	5	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of FHD continues to require a combination of clinical evaluation and a series of diagnostic tests , often requiring reevaluations over time .
	manualset3
146743	1	409535	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of RS was based on the combination of dermatological and articular alterations .
	manualset3
146744	2	409535	5	NULL	NULL	0	NULL	RS 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of RS was based on the combination of dermatological and articular alterations .
	manualset3
146745	3	409535	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of RS was based on the combination of dermatological and articular alterations .
	manualset3
146746	4	409535	5	NULL	NULL	0	NULL	dermatological alterations 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of RS was based on the combination of dermatological and articular alterations .
	manualset3
146747	5	409535	5	NULL	NULL	0	NULL	articular alterations 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of RS was based on the combination of dermatological and articular alterations .
	manualset3
146748	1	409536	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of afferent loop syndrome was confirmed , and the patients were successfully treated by inserting an endoscopic metal stent using a colonoscopic endoscope .
	manualset3
146749	2	409536	5	NULL	NULL	0	NULL	afferent loop syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of afferent loop syndrome was confirmed , and the patients were successfully treated by inserting an endoscopic metal stent using a colonoscopic endoscope .
	manualset3
146750	3	409536	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of afferent loop syndrome was confirmed , and the patients were successfully treated by inserting an endoscopic metal stent using a colonoscopic endoscope .
	manualset3
146751	4	409536	5	NULL	NULL	0	NULL	endoscopic metal stent	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of afferent loop syndrome was confirmed , and the patients were successfully treated by inserting an endoscopic metal stent using a colonoscopic endoscope .
	manualset3
146752	5	409536	5	NULL	NULL	0	NULL	colonoscopic endoscope	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of afferent loop syndrome was confirmed , and the patients were successfully treated by inserting an endoscopic metal stent using a colonoscopic endoscope .
	manualset3
146753	1	409537	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of pulmonary embolism is challenging because lung scanning is nondiagnostic in most patients and because pulmonary angiography is invasive .
	manualset3
146754	2	409537	5	NULL	NULL	0	NULL	pulmonary embolism 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of pulmonary embolism is challenging because lung scanning is nondiagnostic in most patients and because pulmonary angiography is invasive .
	manualset3
146755	3	409537	5	NULL	NULL	0	NULL	lung scanning	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of pulmonary embolism is challenging because lung scanning is nondiagnostic in most patients and because pulmonary angiography is invasive .
	manualset3
146756	4	409537	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of pulmonary embolism is challenging because lung scanning is nondiagnostic in most patients and because pulmonary angiography is invasive .
	manualset3
146757	5	409537	5	NULL	NULL	0	NULL	pulmonary angiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of pulmonary embolism is challenging because lung scanning is nondiagnostic in most patients and because pulmonary angiography is invasive .
	manualset3
146758	1	409538	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of sinus histiocytosis with massive lymphadenopathy ( Rosai and Dorfman , 1969 ) was retained on account of a massive hyperplasia of foamy histiocytes with PAS + inclusions , lipidic storage and hemocytophagy in the sinuses and cords of the lymph nodes .
	manualset3
146759	2	409538	5	NULL	NULL	0	NULL	sinus histiocytosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of sinus histiocytosis with massive lymphadenopathy ( Rosai and Dorfman , 1969 ) was retained on account of a massive hyperplasia of foamy histiocytes with PAS + inclusions , lipidic storage and hemocytophagy in the sinuses and cords of the lymph nodes .
	manualset3
146760	3	409538	5	NULL	NULL	0	NULL	massive lymphadenopathy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of sinus histiocytosis with massive lymphadenopathy ( Rosai and Dorfman , 1969 ) was retained on account of a massive hyperplasia of foamy histiocytes with PAS + inclusions , lipidic storage and hemocytophagy in the sinuses and cords of the lymph nodes .
	manualset3
146761	4	409538	5	NULL	NULL	0	NULL	Rosai 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of sinus histiocytosis with massive lymphadenopathy ( Rosai and Dorfman , 1969 ) was retained on account of a massive hyperplasia of foamy histiocytes with PAS + inclusions , lipidic storage and hemocytophagy in the sinuses and cords of the lymph nodes .
	manualset3
146762	5	409538	5	NULL	NULL	0	NULL	Dorfman 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of sinus histiocytosis with massive lymphadenopathy ( Rosai and Dorfman , 1969 ) was retained on account of a massive hyperplasia of foamy histiocytes with PAS + inclusions , lipidic storage and hemocytophagy in the sinuses and cords of the lymph nodes .
	manualset3
146763	6	409538	5	NULL	NULL	0	NULL	1969 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of sinus histiocytosis with massive lymphadenopathy ( Rosai and Dorfman , 1969 ) was retained on account of a massive hyperplasia of foamy histiocytes with PAS + inclusions , lipidic storage and hemocytophagy in the sinuses and cords of the lymph nodes .
	manualset3
146764	7	409538	5	NULL	NULL	0	NULL	account 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of sinus histiocytosis with massive lymphadenopathy ( Rosai and Dorfman , 1969 ) was retained on account of a massive hyperplasia of foamy histiocytes with PAS + inclusions , lipidic storage and hemocytophagy in the sinuses and cords of the lymph nodes .
	manualset3
146765	8	409538	5	NULL	NULL	0	NULL	massive hyperplasia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of sinus histiocytosis with massive lymphadenopathy ( Rosai and Dorfman , 1969 ) was retained on account of a massive hyperplasia of foamy histiocytes with PAS + inclusions , lipidic storage and hemocytophagy in the sinuses and cords of the lymph nodes .
	manualset3
146766	9	409538	5	NULL	NULL	0	NULL	foamy histiocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of sinus histiocytosis with massive lymphadenopathy ( Rosai and Dorfman , 1969 ) was retained on account of a massive hyperplasia of foamy histiocytes with PAS + inclusions , lipidic storage and hemocytophagy in the sinuses and cords of the lymph nodes .
	manualset3
146767	10	409538	5	NULL	NULL	0	NULL	PAS + inclusions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of sinus histiocytosis with massive lymphadenopathy ( Rosai and Dorfman , 1969 ) was retained on account of a massive hyperplasia of foamy histiocytes with PAS + inclusions , lipidic storage and hemocytophagy in the sinuses and cords of the lymph nodes .
	manualset3
146768	11	409538	5	NULL	NULL	0	NULL	lipidic storage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of sinus histiocytosis with massive lymphadenopathy ( Rosai and Dorfman , 1969 ) was retained on account of a massive hyperplasia of foamy histiocytes with PAS + inclusions , lipidic storage and hemocytophagy in the sinuses and cords of the lymph nodes .
	manualset3
146769	12	409538	5	NULL	NULL	0	NULL	hemocytophagy 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of sinus histiocytosis with massive lymphadenopathy ( Rosai and Dorfman , 1969 ) was retained on account of a massive hyperplasia of foamy histiocytes with PAS + inclusions , lipidic storage and hemocytophagy in the sinuses and cords of the lymph nodes .
	manualset3
146770	13	409538	5	NULL	NULL	0	NULL	sinuses 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of sinus histiocytosis with massive lymphadenopathy ( Rosai and Dorfman , 1969 ) was retained on account of a massive hyperplasia of foamy histiocytes with PAS + inclusions , lipidic storage and hemocytophagy in the sinuses and cords of the lymph nodes .
	manualset3
146771	14	409538	5	NULL	NULL	0	NULL	cords of the lymph nodes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis of sinus histiocytosis with massive lymphadenopathy ( Rosai and Dorfman , 1969 ) was retained on account of a massive hyperplasia of foamy histiocytes with PAS + inclusions , lipidic storage and hemocytophagy in the sinuses and cords of the lymph nodes .
	manualset3
146772	1	409539	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis was determined as congenital mid-ureteral stricture because the ureter tapered smoothly from 25 mm to 5 mm in diameter at the stenotic site .
	manualset3
146773	2	409539	5	NULL	NULL	0	NULL	congenital mid-ureteral stricture	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis was determined as congenital mid-ureteral stricture because the ureter tapered smoothly from 25 mm to 5 mm in diameter at the stenotic site .
	manualset3
146774	3	409539	5	NULL	NULL	0	NULL	ureter 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis was determined as congenital mid-ureteral stricture because the ureter tapered smoothly from 25 mm to 5 mm in diameter at the stenotic site .
	manualset3
146775	4	409539	5	NULL	NULL	0	NULL	 25 mm to 5 mm 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis was determined as congenital mid-ureteral stricture because the ureter tapered smoothly from 25 mm to 5 mm in diameter at the stenotic site .
	manualset3
146776	5	409539	5	NULL	NULL	0	NULL	diameter 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis was determined as congenital mid-ureteral stricture because the ureter tapered smoothly from 25 mm to 5 mm in diameter at the stenotic site .
	manualset3
146777	6	409539	5	NULL	NULL	0	NULL	stenotic site 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis was determined as congenital mid-ureteral stricture because the ureter tapered smoothly from 25 mm to 5 mm in diameter at the stenotic site .
	manualset3
146778	1	409540	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis was initially suspected because of the characteristic clinical features and the strong family history of convulsions .
	manualset3
146779	2	409540	5	NULL	NULL	0	NULL	characteristic clinical features 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis was initially suspected because of the characteristic clinical features and the strong family history of convulsions .
	manualset3
146780	3	409540	5	NULL	NULL	0	NULL	strong family history	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis was initially suspected because of the characteristic clinical features and the strong family history of convulsions .
	manualset3
146781	4	409540	5	NULL	NULL	0	NULL	convulsions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis was initially suspected because of the characteristic clinical features and the strong family history of convulsions .
	manualset3
146782	1	409541	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis was made as result of stool and skin biopsy culture .
	manualset3
146783	2	409541	5	NULL	NULL	0	NULL	result 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis was made as result of stool and skin biopsy culture .
	manualset3
146784	3	409541	5	NULL	NULL	0	NULL	stool culture 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis was made as result of stool and skin biopsy culture .
	manualset3
146785	4	409541	5	NULL	NULL	0	NULL	skin biopsy culture 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis was made as result of stool and skin biopsy culture .
	manualset3
146786	1	409542	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis was made during a severe hypertensive crisis .
	manualset3
146787	2	409542	5	NULL	NULL	0	NULL	severe hypertensive crisis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis was made during a severe hypertensive crisis .
	manualset3
146788	1	409543	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis was made during surgery in one case and at colonoscopy in the other .
	manualset3
146789	2	409543	5	NULL	NULL	0	NULL	surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis was made during surgery in one case and at colonoscopy in the other .
	manualset3
146790	3	409543	5	NULL	NULL	0	NULL	one case	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis was made during surgery in one case and at colonoscopy in the other .
	manualset3
146791	4	409543	5	NULL	NULL	0	NULL	colonoscopy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis was made during surgery in one case and at colonoscopy in the other .
	manualset3
146792	1	409544	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis was made on the basis of trephine biopsy and fine needle aspiration biopsy of the spleen .
	manualset3
146793	2	409544	5	NULL	NULL	0	NULL	trephine biopsy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis was made on the basis of trephine biopsy and fine needle aspiration biopsy of the spleen .
	manualset3
146794	3	409544	5	NULL	NULL	0	NULL	fine needle aspiration biopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis was made on the basis of trephine biopsy and fine needle aspiration biopsy of the spleen .
	manualset3
146795	4	409544	5	NULL	NULL	0	NULL	spleen 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis was made on the basis of trephine biopsy and fine needle aspiration biopsy of the spleen .
	manualset3
146796	1	409545	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis was made on the result of histopathological examination of excised tuberculoma .
	manualset3
146797	2	409545	5	NULL	NULL	0	NULL	result 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis was made on the result of histopathological examination of excised tuberculoma .
	manualset3
146798	3	409545	5	NULL	NULL	NULL	NULL	histopathological examination	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The diagnosis was made on the result of histopathological examination of excised tuberculoma .
	manualset3
146799	4	409545	5	NULL	NULL	0	NULL	excised tuberculoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis was made on the result of histopathological examination of excised tuberculoma .
	manualset3
146800	1	409546	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis was verified by histological investigation of the operative specimen .
	manualset3
146801	2	409546	5	NULL	NULL	0	NULL	histological investigation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis was verified by histological investigation of the operative specimen .
	manualset3
146802	3	409546	5	NULL	NULL	0	NULL	operative specimen	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnosis was verified by histological investigation of the operative specimen .
	manualset3
146803	1	409547	5	NULL	NULL	0	NULL	diagnostic approach	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnostic approach to the patient with suspected mitochondrial disease entails a detailed personal and family history , careful ophthalmic , neurologic , and systemic examination , directed investigations , and attention to potentially life-threatening sequelae .
	manualset3
146804	2	409547	5	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnostic approach to the patient with suspected mitochondrial disease entails a detailed personal and family history , careful ophthalmic , neurologic , and systemic examination , directed investigations , and attention to potentially life-threatening sequelae .
	manualset3
146805	3	409547	5	NULL	NULL	0	NULL	mitochondrial disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnostic approach to the patient with suspected mitochondrial disease entails a detailed personal and family history , careful ophthalmic , neurologic , and systemic examination , directed investigations , and attention to potentially life-threatening sequelae .
	manualset3
146806	4	409547	5	NULL	NULL	0	NULL	personal history 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnostic approach to the patient with suspected mitochondrial disease entails a detailed personal and family history , careful ophthalmic , neurologic , and systemic examination , directed investigations , and attention to potentially life-threatening sequelae .
	manualset3
146807	5	409547	5	NULL	NULL	0	NULL	family history 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnostic approach to the patient with suspected mitochondrial disease entails a detailed personal and family history , careful ophthalmic , neurologic , and systemic examination , directed investigations , and attention to potentially life-threatening sequelae .
	manualset3
146808	6	409547	5	NULL	NULL	0	NULL	ophthalmic examination 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnostic approach to the patient with suspected mitochondrial disease entails a detailed personal and family history , careful ophthalmic , neurologic , and systemic examination , directed investigations , and attention to potentially life-threatening sequelae .
	manualset3
146809	7	409547	5	NULL	NULL	0	NULL	neurologic examination 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnostic approach to the patient with suspected mitochondrial disease entails a detailed personal and family history , careful ophthalmic , neurologic , and systemic examination , directed investigations , and attention to potentially life-threatening sequelae .
	manualset3
146810	8	409547	5	NULL	NULL	0	NULL	systemic examination 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnostic approach to the patient with suspected mitochondrial disease entails a detailed personal and family history , careful ophthalmic , neurologic , and systemic examination , directed investigations , and attention to potentially life-threatening sequelae .
	manualset3
146811	9	409547	5	NULL	NULL	0	NULL	directed investigations 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnostic approach to the patient with suspected mitochondrial disease entails a detailed personal and family history , careful ophthalmic , neurologic , and systemic examination , directed investigations , and attention to potentially life-threatening sequelae .
	manualset3
146812	10	409547	5	NULL	NULL	0	NULL	attention 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnostic approach to the patient with suspected mitochondrial disease entails a detailed personal and family history , careful ophthalmic , neurologic , and systemic examination , directed investigations , and attention to potentially life-threatening sequelae .
	manualset3
146813	11	409547	5	NULL	NULL	0	NULL	potentially life-threatening sequelae	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The diagnostic approach to the patient with suspected mitochondrial disease entails a detailed personal and family history , careful ophthalmic , neurologic , and systemic examination , directed investigations , and attention to potentially life-threatening sequelae .
	manualset3
146814	1	409548	5	NULL	NULL	0	NULL	single amino acid substitution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A single amino acid substitution in GAD65 at position 401 ( leucine to proline ) and representing the analogous GAD67 sequence in this region significantly reduced the peptide 's inhibitory effect .
	manualset3
146815	2	409548	5	NULL	NULL	0	NULL	GAD65 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A single amino acid substitution in GAD65 at position 401 ( leucine to proline ) and representing the analogous GAD67 sequence in this region significantly reduced the peptide 's inhibitory effect .
	manualset3
146816	3	409548	5	NULL	NULL	0	NULL	position 401	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A single amino acid substitution in GAD65 at position 401 ( leucine to proline ) and representing the analogous GAD67 sequence in this region significantly reduced the peptide 's inhibitory effect .
	manualset3
146817	4	409548	5	NULL	NULL	0	NULL	leucine 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A single amino acid substitution in GAD65 at position 401 ( leucine to proline ) and representing the analogous GAD67 sequence in this region significantly reduced the peptide 's inhibitory effect .
	manualset3
146818	5	409548	5	NULL	NULL	0	NULL	proline 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A single amino acid substitution in GAD65 at position 401 ( leucine to proline ) and representing the analogous GAD67 sequence in this region significantly reduced the peptide 's inhibitory effect .
	manualset3
146819	6	409548	5	NULL	NULL	0	NULL	analogous GAD67 sequence 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A single amino acid substitution in GAD65 at position 401 ( leucine to proline ) and representing the analogous GAD67 sequence in this region significantly reduced the peptide 's inhibitory effect .
	manualset3
146820	7	409548	5	NULL	NULL	0	NULL	region 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A single amino acid substitution in GAD65 at position 401 ( leucine to proline ) and representing the analogous GAD67 sequence in this region significantly reduced the peptide 's inhibitory effect .
	manualset3
146821	8	409548	5	NULL	NULL	0	NULL	inhibitory effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A single amino acid substitution in GAD65 at position 401 ( leucine to proline ) and representing the analogous GAD67 sequence in this region significantly reduced the peptide 's inhibitory effect .
	manualset3
146822	1	409549	5	NULL	NULL	0	NULL	diameter 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The diameter of the anterior choroidal artery was 0.94 mm on average ( 0.7-1 .2 ) and the average distance from the posterior communicating artery was 5.3 mm ( 3.8-8 mm ) ; its distance to the bifurcation of the carotid was found to be 4.0 mm on average ( 2.2-8 mm ) .
	manualset3
146823	2	409549	5	NULL	NULL	0	NULL	anterior choroidal artery 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The diameter of the anterior choroidal artery was 0.94 mm on average ( 0.7-1 .2 ) and the average distance from the posterior communicating artery was 5.3 mm ( 3.8-8 mm ) ; its distance to the bifurcation of the carotid was found to be 4.0 mm on average ( 2.2-8 mm ) .
	manualset3
146824	3	409549	5	NULL	NULL	0	NULL	0.94 mm on average ( 0.7-1 .2 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The diameter of the anterior choroidal artery was 0.94 mm on average ( 0.7-1 .2 ) and the average distance from the posterior communicating artery was 5.3 mm ( 3.8-8 mm ) ; its distance to the bifurcation of the carotid was found to be 4.0 mm on average ( 2.2-8 mm ) .
	manualset3
146825	4	409549	5	NULL	NULL	0	NULL	average distance	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The diameter of the anterior choroidal artery was 0.94 mm on average ( 0.7-1 .2 ) and the average distance from the posterior communicating artery was 5.3 mm ( 3.8-8 mm ) ; its distance to the bifurcation of the carotid was found to be 4.0 mm on average ( 2.2-8 mm ) .
	manualset3
146826	5	409549	5	NULL	NULL	0	NULL	posterior communicating artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The diameter of the anterior choroidal artery was 0.94 mm on average ( 0.7-1 .2 ) and the average distance from the posterior communicating artery was 5.3 mm ( 3.8-8 mm ) ; its distance to the bifurcation of the carotid was found to be 4.0 mm on average ( 2.2-8 mm ) .
	manualset3
146827	6	409549	5	NULL	NULL	0	NULL	5.3 mm ( 3.8-8 mm )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The diameter of the anterior choroidal artery was 0.94 mm on average ( 0.7-1 .2 ) and the average distance from the posterior communicating artery was 5.3 mm ( 3.8-8 mm ) ; its distance to the bifurcation of the carotid was found to be 4.0 mm on average ( 2.2-8 mm ) .
	manualset3
146828	7	409549	5	NULL	NULL	0	NULL	distance 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The diameter of the anterior choroidal artery was 0.94 mm on average ( 0.7-1 .2 ) and the average distance from the posterior communicating artery was 5.3 mm ( 3.8-8 mm ) ; its distance to the bifurcation of the carotid was found to be 4.0 mm on average ( 2.2-8 mm ) .
	manualset3
146829	8	409549	5	NULL	NULL	0	NULL	bifurcation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The diameter of the anterior choroidal artery was 0.94 mm on average ( 0.7-1 .2 ) and the average distance from the posterior communicating artery was 5.3 mm ( 3.8-8 mm ) ; its distance to the bifurcation of the carotid was found to be 4.0 mm on average ( 2.2-8 mm ) .
	manualset3
146830	9	409549	5	NULL	NULL	0	NULL	carotid 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The diameter of the anterior choroidal artery was 0.94 mm on average ( 0.7-1 .2 ) and the average distance from the posterior communicating artery was 5.3 mm ( 3.8-8 mm ) ; its distance to the bifurcation of the carotid was found to be 4.0 mm on average ( 2.2-8 mm ) .
	manualset3
146831	10	409549	5	NULL	NULL	0	NULL	 4.0 mm on average ( 2.2-8 mm )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The diameter of the anterior choroidal artery was 0.94 mm on average ( 0.7-1 .2 ) and the average distance from the posterior communicating artery was 5.3 mm ( 3.8-8 mm ) ; its distance to the bifurcation of the carotid was found to be 4.0 mm on average ( 2.2-8 mm ) .
	manualset3
146832	1	409550	5	NULL	NULL	NULL	NULL	diameter ranges	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The diameter ranges for the undoped , N-doped ( pyridine ) , N-doped ( NH ( 3 ) ) , and B-doped DWNTs are 0.73-2 .20 , 0.74-2 .30 , 0.73-2 .32 , and 0.74-2 .36 nm , respectively , the boron-doped DWNTs giving rise to a high proportion of the large diameter DWNTs .
	manualset3
146839	2	409550	5	NULL	NULL	0	NULL	undoped DWNTs 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The diameter ranges for the undoped , N-doped ( pyridine ) , N-doped ( NH ( 3 ) ) , and B-doped DWNTs are 0.73-2 .20 , 0.74-2 .30 , 0.73-2 .32 , and 0.74-2 .36 nm , respectively , the boron-doped DWNTs giving rise to a high proportion of the large diameter DWNTs .
	manualset3
146840	3	409550	5	NULL	NULL	0	NULL	N-doped ( pyridine ) DWNTs 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The diameter ranges for the undoped , N-doped ( pyridine ) , N-doped ( NH ( 3 ) ) , and B-doped DWNTs are 0.73-2 .20 , 0.74-2 .30 , 0.73-2 .32 , and 0.74-2 .36 nm , respectively , the boron-doped DWNTs giving rise to a high proportion of the large diameter DWNTs .
	manualset3
146841	4	409550	5	NULL	NULL	0	NULL	N-doped ( NH ( 3 ) ) DWNTs 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The diameter ranges for the undoped , N-doped ( pyridine ) , N-doped ( NH ( 3 ) ) , and B-doped DWNTs are 0.73-2 .20 , 0.74-2 .30 , 0.73-2 .32 , and 0.74-2 .36 nm , respectively , the boron-doped DWNTs giving rise to a high proportion of the large diameter DWNTs .
	manualset3
146842	5	409550	5	NULL	NULL	0	NULL	B-doped DWNTs 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The diameter ranges for the undoped , N-doped ( pyridine ) , N-doped ( NH ( 3 ) ) , and B-doped DWNTs are 0.73-2 .20 , 0.74-2 .30 , 0.73-2 .32 , and 0.74-2 .36 nm , respectively , the boron-doped DWNTs giving rise to a high proportion of the large diameter DWNTs .
	manualset3
146843	6	409550	5	NULL	NULL	0	NULL	0.73-2 .20 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The diameter ranges for the undoped , N-doped ( pyridine ) , N-doped ( NH ( 3 ) ) , and B-doped DWNTs are 0.73-2 .20 , 0.74-2 .30 , 0.73-2 .32 , and 0.74-2 .36 nm , respectively , the boron-doped DWNTs giving rise to a high proportion of the large diameter DWNTs .
	manualset3
146844	7	409550	5	NULL	NULL	0	NULL	0.74-2 .30 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The diameter ranges for the undoped , N-doped ( pyridine ) , N-doped ( NH ( 3 ) ) , and B-doped DWNTs are 0.73-2 .20 , 0.74-2 .30 , 0.73-2 .32 , and 0.74-2 .36 nm , respectively , the boron-doped DWNTs giving rise to a high proportion of the large diameter DWNTs .
	manualset3
146845	8	409550	5	NULL	NULL	0	NULL	0.73-2 .32 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The diameter ranges for the undoped , N-doped ( pyridine ) , N-doped ( NH ( 3 ) ) , and B-doped DWNTs are 0.73-2 .20 , 0.74-2 .30 , 0.73-2 .32 , and 0.74-2 .36 nm , respectively , the boron-doped DWNTs giving rise to a high proportion of the large diameter DWNTs .
	manualset3
146846	9	409550	5	NULL	NULL	0	NULL	0.74-2 .36 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The diameter ranges for the undoped , N-doped ( pyridine ) , N-doped ( NH ( 3 ) ) , and B-doped DWNTs are 0.73-2 .20 , 0.74-2 .30 , 0.73-2 .32 , and 0.74-2 .36 nm , respectively , the boron-doped DWNTs giving rise to a high proportion of the large diameter DWNTs .
	manualset3
146847	10	409550	5	NULL	NULL	0	NULL	boron-doped DWNTs 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The diameter ranges for the undoped , N-doped ( pyridine ) , N-doped ( NH ( 3 ) ) , and B-doped DWNTs are 0.73-2 .20 , 0.74-2 .30 , 0.73-2 .32 , and 0.74-2 .36 nm , respectively , the boron-doped DWNTs giving rise to a high proportion of the large diameter DWNTs .
	manualset3
146848	11	409550	5	NULL	NULL	0	NULL	high proportion	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The diameter ranges for the undoped , N-doped ( pyridine ) , N-doped ( NH ( 3 ) ) , and B-doped DWNTs are 0.73-2 .20 , 0.74-2 .30 , 0.73-2 .32 , and 0.74-2 .36 nm , respectively , the boron-doped DWNTs giving rise to a high proportion of the large diameter DWNTs .
	manualset3
146849	12	409550	5	NULL	NULL	0	NULL	large diameter DWNTs	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The diameter ranges for the undoped , N-doped ( pyridine ) , N-doped ( NH ( 3 ) ) , and B-doped DWNTs are 0.73-2 .20 , 0.74-2 .30 , 0.73-2 .32 , and 0.74-2 .36 nm , respectively , the boron-doped DWNTs giving rise to a high proportion of the large diameter DWNTs .
	manualset3
146850	1	409551	5	NULL	NULL	NULL	NULL	dietary approaches to stop hypertension ( DASH ) clinical trial	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The dietary approaches to stop hypertension ( DASH ) clinical trial : implications for lifestyle modifications in the treatment of hypertensive patients .
	manualset3
146851	2	409551	5	NULL	NULL	0	NULL	implications 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dietary approaches to stop hypertension ( DASH ) clinical trial : implications for lifestyle modifications in the treatment of hypertensive patients .
	manualset3
146852	3	409551	5	NULL	NULL	0	NULL	lifestyle modifications 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dietary approaches to stop hypertension ( DASH ) clinical trial : implications for lifestyle modifications in the treatment of hypertensive patients .
	manualset3
146853	4	409551	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The dietary approaches to stop hypertension ( DASH ) clinical trial : implications for lifestyle modifications in the treatment of hypertensive patients .
	manualset3
146854	5	409551	5	NULL	NULL	0	NULL	hypertensive patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The dietary approaches to stop hypertension ( DASH ) clinical trial : implications for lifestyle modifications in the treatment of hypertensive patients .
	manualset3
146855	1	409552	5	NULL	NULL	0	NULL	dietary intake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dietary intake of micronutrients and serum micronutrient status have been topics of concern in relation to human immunodeficiency virus ( HIV ) progression .
	manualset3
146856	2	409552	5	NULL	NULL	0	NULL	micronutrients 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The dietary intake of micronutrients and serum micronutrient status have been topics of concern in relation to human immunodeficiency virus ( HIV ) progression .
	manualset3
146857	3	409552	5	NULL	NULL	0	NULL	serum micronutrient status 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dietary intake of micronutrients and serum micronutrient status have been topics of concern in relation to human immunodeficiency virus ( HIV ) progression .
	manualset3
146858	4	409552	5	NULL	NULL	0	NULL	topics of concern	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The dietary intake of micronutrients and serum micronutrient status have been topics of concern in relation to human immunodeficiency virus ( HIV ) progression .
	manualset3
146859	5	409552	5	NULL	NULL	0	NULL	relation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The dietary intake of micronutrients and serum micronutrient status have been topics of concern in relation to human immunodeficiency virus ( HIV ) progression .
	manualset3
146860	6	409552	5	NULL	NULL	0	NULL	human immunodeficiency virus ( HIV ) progression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The dietary intake of micronutrients and serum micronutrient status have been topics of concern in relation to human immunodeficiency virus ( HIV ) progression .
	manualset3
146861	1	409553	5	NULL	NULL	0	NULL	difference 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The difference between the most and the least toxic components was approximately 17 , 000-fold and 1 , 000 , 000-fold for the mg/L and mmol/L EC50 data , respectively .
	manualset3
146862	2	409553	5	NULL	NULL	0	NULL	toxic components 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The difference between the most and the least toxic components was approximately 17 , 000-fold and 1 , 000 , 000-fold for the mg/L and mmol/L EC50 data , respectively .
	manualset3
146863	3	409553	5	NULL	NULL	0	NULL	17 , 000-fold for mg/L data	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The difference between the most and the least toxic components was approximately 17 , 000-fold and 1 , 000 , 000-fold for the mg/L and mmol/L EC50 data , respectively .
	manualset3
146864	4	409553	5	NULL	NULL	0	NULL	1 , 000 , 000-fold for  mmol/L EC50 data 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The difference between the most and the least toxic components was approximately 17 , 000-fold and 1 , 000 , 000-fold for the mg/L and mmol/L EC50 data , respectively .
	manualset3
146865	1	409554	5	NULL	NULL	0	NULL	difference 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The difference between winter and summer was confirmed the following year in LD conditions .
	manualset3
146866	2	409554	5	NULL	NULL	0	NULL	winter 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The difference between winter and summer was confirmed the following year in LD conditions .
	manualset3
146867	3	409554	5	NULL	NULL	0	NULL	summer 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The difference between winter and summer was confirmed the following year in LD conditions .
	manualset3
146868	4	409554	5	NULL	NULL	0	NULL	year 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The difference between winter and summer was confirmed the following year in LD conditions .
	manualset3
146869	5	409554	5	NULL	NULL	0	NULL	LD conditions	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The difference between winter and summer was confirmed the following year in LD conditions .
	manualset3
146870	1	409555	5	NULL	NULL	0	NULL	difference 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The difference can be definitely explained by the influence of butyl scopolamine and the high-pressure injection of the contrast medium into the bile duct system .
	manualset3
146871	2	409555	5	NULL	NULL	0	NULL	influence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The difference can be definitely explained by the influence of butyl scopolamine and the high-pressure injection of the contrast medium into the bile duct system .
	manualset3
146872	3	409555	5	NULL	NULL	0	NULL	butyl scopolamine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The difference can be definitely explained by the influence of butyl scopolamine and the high-pressure injection of the contrast medium into the bile duct system .
	manualset3
146873	4	409555	5	NULL	NULL	0	NULL	high-pressure injection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The difference can be definitely explained by the influence of butyl scopolamine and the high-pressure injection of the contrast medium into the bile duct system .
	manualset3
146874	5	409555	5	NULL	NULL	0	NULL	contrast medium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The difference can be definitely explained by the influence of butyl scopolamine and the high-pressure injection of the contrast medium into the bile duct system .
	manualset3
146875	6	409555	5	NULL	NULL	0	NULL	bile duct system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The difference can be definitely explained by the influence of butyl scopolamine and the high-pressure injection of the contrast medium into the bile duct system .
	manualset3
146876	1	409556	5	NULL	NULL	0	NULL	difference 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The difference in plaque pH between miswak extract and water rinse was statistically significant at 30 min ( p & lt ; 0.001 ) .
	manualset3
146877	2	409556	5	NULL	NULL	0	NULL	plaque pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The difference in plaque pH between miswak extract and water rinse was statistically significant at 30 min ( p & lt ; 0.001 ) .
	manualset3
146878	3	409556	5	NULL	NULL	0	NULL	miswak extract	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The difference in plaque pH between miswak extract and water rinse was statistically significant at 30 min ( p & lt ; 0.001 ) .
	manualset3
146879	4	409556	5	NULL	NULL	0	NULL	water rinse 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The difference in plaque pH between miswak extract and water rinse was statistically significant at 30 min ( p & lt ; 0.001 ) .
	manualset3
146880	5	409556	5	NULL	NULL	0	NULL	30 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The difference in plaque pH between miswak extract and water rinse was statistically significant at 30 min ( p & lt ; 0.001 ) .
	manualset3
146881	6	409556	5	NULL	NULL	0	NULL	p & lt ; 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The difference in plaque pH between miswak extract and water rinse was statistically significant at 30 min ( p & lt ; 0.001 ) .
	manualset3
146882	1	409557	5	NULL	NULL	0	NULL	 single dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A single dose of CLARI-MINO , with or without OFLO , displayed bactericidal activity as great as that of 4 weeks of daily treatment with dapsone ( DDS ) plus clofazimine ( CLO ) ; thus , intermittent CLARI-MINO , with or without OFLO , may replace DDS and CLO of the standard multidrug regimen , and these will become regimens that can be administered monthly and under full supervision .
	manualset3
146883	2	409557	5	NULL	NULL	0	NULL	CLARI-MINO	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A single dose of CLARI-MINO , with or without OFLO , displayed bactericidal activity as great as that of 4 weeks of daily treatment with dapsone ( DDS ) plus clofazimine ( CLO ) ; thus , intermittent CLARI-MINO , with or without OFLO , may replace DDS and CLO of the standard multidrug regimen , and these will become regimens that can be administered monthly and under full supervision .
	manualset3
146884	3	409557	5	NULL	NULL	0	NULL	OFLO 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A single dose of CLARI-MINO , with or without OFLO , displayed bactericidal activity as great as that of 4 weeks of daily treatment with dapsone ( DDS ) plus clofazimine ( CLO ) ; thus , intermittent CLARI-MINO , with or without OFLO , may replace DDS and CLO of the standard multidrug regimen , and these will become regimens that can be administered monthly and under full supervision .
	manualset3
146885	4	409557	5	NULL	NULL	0	NULL	bactericidal activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A single dose of CLARI-MINO , with or without OFLO , displayed bactericidal activity as great as that of 4 weeks of daily treatment with dapsone ( DDS ) plus clofazimine ( CLO ) ; thus , intermittent CLARI-MINO , with or without OFLO , may replace DDS and CLO of the standard multidrug regimen , and these will become regimens that can be administered monthly and under full supervision .
	manualset3
146886	5	409557	5	NULL	NULL	0	NULL	4 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A single dose of CLARI-MINO , with or without OFLO , displayed bactericidal activity as great as that of 4 weeks of daily treatment with dapsone ( DDS ) plus clofazimine ( CLO ) ; thus , intermittent CLARI-MINO , with or without OFLO , may replace DDS and CLO of the standard multidrug regimen , and these will become regimens that can be administered monthly and under full supervision .
	manualset3
146887	6	409557	5	NULL	NULL	0	NULL	daily treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A single dose of CLARI-MINO , with or without OFLO , displayed bactericidal activity as great as that of 4 weeks of daily treatment with dapsone ( DDS ) plus clofazimine ( CLO ) ; thus , intermittent CLARI-MINO , with or without OFLO , may replace DDS and CLO of the standard multidrug regimen , and these will become regimens that can be administered monthly and under full supervision .
	manualset3
146888	7	409557	5	NULL	NULL	0	NULL	dapsone ( DDS )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A single dose of CLARI-MINO , with or without OFLO , displayed bactericidal activity as great as that of 4 weeks of daily treatment with dapsone ( DDS ) plus clofazimine ( CLO ) ; thus , intermittent CLARI-MINO , with or without OFLO , may replace DDS and CLO of the standard multidrug regimen , and these will become regimens that can be administered monthly and under full supervision .
	manualset3
146889	8	409557	5	NULL	NULL	0	NULL	 clofazimine ( CLO )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A single dose of CLARI-MINO , with or without OFLO , displayed bactericidal activity as great as that of 4 weeks of daily treatment with dapsone ( DDS ) plus clofazimine ( CLO ) ; thus , intermittent CLARI-MINO , with or without OFLO , may replace DDS and CLO of the standard multidrug regimen , and these will become regimens that can be administered monthly and under full supervision .
	manualset3
146890	9	409557	5	NULL	NULL	0	NULL	intermittent CLARI-MINO	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A single dose of CLARI-MINO , with or without OFLO , displayed bactericidal activity as great as that of 4 weeks of daily treatment with dapsone ( DDS ) plus clofazimine ( CLO ) ; thus , intermittent CLARI-MINO , with or without OFLO , may replace DDS and CLO of the standard multidrug regimen , and these will become regimens that can be administered monthly and under full supervision .
	manualset3
146891	10	409557	5	NULL	NULL	0	NULL	OFLO 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A single dose of CLARI-MINO , with or without OFLO , displayed bactericidal activity as great as that of 4 weeks of daily treatment with dapsone ( DDS ) plus clofazimine ( CLO ) ; thus , intermittent CLARI-MINO , with or without OFLO , may replace DDS and CLO of the standard multidrug regimen , and these will become regimens that can be administered monthly and under full supervision .
	manualset3
146892	11	409557	5	NULL	NULL	0	NULL	DDS 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A single dose of CLARI-MINO , with or without OFLO , displayed bactericidal activity as great as that of 4 weeks of daily treatment with dapsone ( DDS ) plus clofazimine ( CLO ) ; thus , intermittent CLARI-MINO , with or without OFLO , may replace DDS and CLO of the standard multidrug regimen , and these will become regimens that can be administered monthly and under full supervision .
	manualset3
146893	12	409557	5	NULL	NULL	0	NULL	CLO 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A single dose of CLARI-MINO , with or without OFLO , displayed bactericidal activity as great as that of 4 weeks of daily treatment with dapsone ( DDS ) plus clofazimine ( CLO ) ; thus , intermittent CLARI-MINO , with or without OFLO , may replace DDS and CLO of the standard multidrug regimen , and these will become regimens that can be administered monthly and under full supervision .
	manualset3
146894	13	409557	5	NULL	NULL	0	NULL	standard multidrug regimen	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A single dose of CLARI-MINO , with or without OFLO , displayed bactericidal activity as great as that of 4 weeks of daily treatment with dapsone ( DDS ) plus clofazimine ( CLO ) ; thus , intermittent CLARI-MINO , with or without OFLO , may replace DDS and CLO of the standard multidrug regimen , and these will become regimens that can be administered monthly and under full supervision .
	manualset3
146895	14	409557	5	NULL	NULL	0	NULL	regimens 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A single dose of CLARI-MINO , with or without OFLO , displayed bactericidal activity as great as that of 4 weeks of daily treatment with dapsone ( DDS ) plus clofazimine ( CLO ) ; thus , intermittent CLARI-MINO , with or without OFLO , may replace DDS and CLO of the standard multidrug regimen , and these will become regimens that can be administered monthly and under full supervision .
	manualset3
146896	15	409557	5	NULL	NULL	0	NULL	monthly 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A single dose of CLARI-MINO , with or without OFLO , displayed bactericidal activity as great as that of 4 weeks of daily treatment with dapsone ( DDS ) plus clofazimine ( CLO ) ; thus , intermittent CLARI-MINO , with or without OFLO , may replace DDS and CLO of the standard multidrug regimen , and these will become regimens that can be administered monthly and under full supervision .
	manualset3
146897	16	409557	5	NULL	NULL	0	NULL	full supervision	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A single dose of CLARI-MINO , with or without OFLO , displayed bactericidal activity as great as that of 4 weeks of daily treatment with dapsone ( DDS ) plus clofazimine ( CLO ) ; thus , intermittent CLARI-MINO , with or without OFLO , may replace DDS and CLO of the standard multidrug regimen , and these will become regimens that can be administered monthly and under full supervision .
	manualset3
146898	1	409558	5	NULL	NULL	0	NULL	difference 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The difference in plasma cholesterol between the two phenotypic groups was in part due to a higher buoyant LDL production rate in Lpb5 .1 pigs than in Lpb5 .2 pigs .
	manualset3
146899	2	409558	5	NULL	NULL	0	NULL	plasma cholesterol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The difference in plasma cholesterol between the two phenotypic groups was in part due to a higher buoyant LDL production rate in Lpb5 .1 pigs than in Lpb5 .2 pigs .
	manualset3
146900	3	409558	5	NULL	NULL	0	NULL	two phenotypic groups	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The difference in plasma cholesterol between the two phenotypic groups was in part due to a higher buoyant LDL production rate in Lpb5 .1 pigs than in Lpb5 .2 pigs .
	manualset3
146901	4	409558	5	NULL	NULL	0	NULL	higher buoyant LDL production rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The difference in plasma cholesterol between the two phenotypic groups was in part due to a higher buoyant LDL production rate in Lpb5 .1 pigs than in Lpb5 .2 pigs .
	manualset3
146902	5	409558	5	NULL	NULL	0	NULL	Lpb5 .1 pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The difference in plasma cholesterol between the two phenotypic groups was in part due to a higher buoyant LDL production rate in Lpb5 .1 pigs than in Lpb5 .2 pigs .
	manualset3
146903	6	409558	5	NULL	NULL	0	NULL	Lpb5 .2 pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The difference in plasma cholesterol between the two phenotypic groups was in part due to a higher buoyant LDL production rate in Lpb5 .1 pigs than in Lpb5 .2 pigs .
	manualset3
146904	1	409559	5	NULL	NULL	0	NULL	differences 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The differences , which can be resolved , are attributable to two major factors : ( 1 ) NMCUES includes only the civilian noninstitutionalized population , but the other estimates include the institutionalized population and the military ; and ( 2 ) NMCUES indirect cost estimates for the population unable to work include persons who were retired for health reasons in 1979 and 1980 , disabled homemakers , and other persons who were disabled for the entire year 1980 but were not retired for health reasons in 1979 , but the Rice et al. estimates do not include the last two categories in the population unable to work .
	manualset3
146905	2	409559	5	NULL	NULL	0	NULL	two major factors 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The differences , which can be resolved , are attributable to two major factors : ( 1 ) NMCUES includes only the civilian noninstitutionalized population , but the other estimates include the institutionalized population and the military ; and ( 2 ) NMCUES indirect cost estimates for the population unable to work include persons who were retired for health reasons in 1979 and 1980 , disabled homemakers , and other persons who were disabled for the entire year 1980 but were not retired for health reasons in 1979 , but the Rice et al. estimates do not include the last two categories in the population unable to work .
	manualset3
146906	3	409559	5	NULL	NULL	0	NULL	NMCUES 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The differences , which can be resolved , are attributable to two major factors : ( 1 ) NMCUES includes only the civilian noninstitutionalized population , but the other estimates include the institutionalized population and the military ; and ( 2 ) NMCUES indirect cost estimates for the population unable to work include persons who were retired for health reasons in 1979 and 1980 , disabled homemakers , and other persons who were disabled for the entire year 1980 but were not retired for health reasons in 1979 , but the Rice et al. estimates do not include the last two categories in the population unable to work .
	manualset3
146907	4	409559	5	NULL	NULL	0	NULL	civilian noninstitutionalized population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The differences , which can be resolved , are attributable to two major factors : ( 1 ) NMCUES includes only the civilian noninstitutionalized population , but the other estimates include the institutionalized population and the military ; and ( 2 ) NMCUES indirect cost estimates for the population unable to work include persons who were retired for health reasons in 1979 and 1980 , disabled homemakers , and other persons who were disabled for the entire year 1980 but were not retired for health reasons in 1979 , but the Rice et al. estimates do not include the last two categories in the population unable to work .
	manualset3
146908	5	409559	5	NULL	NULL	0	NULL	institutionalized population 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The differences , which can be resolved , are attributable to two major factors : ( 1 ) NMCUES includes only the civilian noninstitutionalized population , but the other estimates include the institutionalized population and the military ; and ( 2 ) NMCUES indirect cost estimates for the population unable to work include persons who were retired for health reasons in 1979 and 1980 , disabled homemakers , and other persons who were disabled for the entire year 1980 but were not retired for health reasons in 1979 , but the Rice et al. estimates do not include the last two categories in the population unable to work .
	manualset3
146909	6	409559	5	NULL	NULL	0	NULL	military 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The differences , which can be resolved , are attributable to two major factors : ( 1 ) NMCUES includes only the civilian noninstitutionalized population , but the other estimates include the institutionalized population and the military ; and ( 2 ) NMCUES indirect cost estimates for the population unable to work include persons who were retired for health reasons in 1979 and 1980 , disabled homemakers , and other persons who were disabled for the entire year 1980 but were not retired for health reasons in 1979 , but the Rice et al. estimates do not include the last two categories in the population unable to work .
	manualset3
146910	7	409559	5	NULL	NULL	0	NULL	NMCUES 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The differences , which can be resolved , are attributable to two major factors : ( 1 ) NMCUES includes only the civilian noninstitutionalized population , but the other estimates include the institutionalized population and the military ; and ( 2 ) NMCUES indirect cost estimates for the population unable to work include persons who were retired for health reasons in 1979 and 1980 , disabled homemakers , and other persons who were disabled for the entire year 1980 but were not retired for health reasons in 1979 , but the Rice et al. estimates do not include the last two categories in the population unable to work .
	manualset3
146911	8	409559	5	NULL	NULL	0	NULL	population 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The differences , which can be resolved , are attributable to two major factors : ( 1 ) NMCUES includes only the civilian noninstitutionalized population , but the other estimates include the institutionalized population and the military ; and ( 2 ) NMCUES indirect cost estimates for the population unable to work include persons who were retired for health reasons in 1979 and 1980 , disabled homemakers , and other persons who were disabled for the entire year 1980 but were not retired for health reasons in 1979 , but the Rice et al. estimates do not include the last two categories in the population unable to work .
	manualset3
146912	9	409559	5	NULL	NULL	NULL	NULL	health reasons	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The differences , which can be resolved , are attributable to two major factors : ( 1 ) NMCUES includes only the civilian noninstitutionalized population , but the other estimates include the institutionalized population and the military ; and ( 2 ) NMCUES indirect cost estimates for the population unable to work include persons who were retired for health reasons in 1979 and 1980 , disabled homemakers , and other persons who were disabled for the entire year 1980 but were not retired for health reasons in 1979 , but the Rice et al. estimates do not include the last two categories in the population unable to work .
	manualset3
146913	10	409559	5	NULL	NULL	0	NULL	1979 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	The differences , which can be resolved , are attributable to two major factors : ( 1 ) NMCUES includes only the civilian noninstitutionalized population , but the other estimates include the institutionalized population and the military ; and ( 2 ) NMCUES indirect cost estimates for the population unable to work include persons who were retired for health reasons in 1979 and 1980 , disabled homemakers , and other persons who were disabled for the entire year 1980 but were not retired for health reasons in 1979 , but the Rice et al. estimates do not include the last two categories in the population unable to work .
	manualset3
146914	11	409559	5	NULL	NULL	0	NULL	1980 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	The differences , which can be resolved , are attributable to two major factors : ( 1 ) NMCUES includes only the civilian noninstitutionalized population , but the other estimates include the institutionalized population and the military ; and ( 2 ) NMCUES indirect cost estimates for the population unable to work include persons who were retired for health reasons in 1979 and 1980 , disabled homemakers , and other persons who were disabled for the entire year 1980 but were not retired for health reasons in 1979 , but the Rice et al. estimates do not include the last two categories in the population unable to work .
	manualset3
146915	12	409559	5	NULL	NULL	0	NULL	disabled homemakers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The differences , which can be resolved , are attributable to two major factors : ( 1 ) NMCUES includes only the civilian noninstitutionalized population , but the other estimates include the institutionalized population and the military ; and ( 2 ) NMCUES indirect cost estimates for the population unable to work include persons who were retired for health reasons in 1979 and 1980 , disabled homemakers , and other persons who were disabled for the entire year 1980 but were not retired for health reasons in 1979 , but the Rice et al. estimates do not include the last two categories in the population unable to work .
	manualset3
146916	13	409559	5	NULL	NULL	0	NULL	persons 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The differences , which can be resolved , are attributable to two major factors : ( 1 ) NMCUES includes only the civilian noninstitutionalized population , but the other estimates include the institutionalized population and the military ; and ( 2 ) NMCUES indirect cost estimates for the population unable to work include persons who were retired for health reasons in 1979 and 1980 , disabled homemakers , and other persons who were disabled for the entire year 1980 but were not retired for health reasons in 1979 , but the Rice et al. estimates do not include the last two categories in the population unable to work .
	manualset3
146917	14	409559	5	NULL	NULL	0	NULL	entire year 1980	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The differences , which can be resolved , are attributable to two major factors : ( 1 ) NMCUES includes only the civilian noninstitutionalized population , but the other estimates include the institutionalized population and the military ; and ( 2 ) NMCUES indirect cost estimates for the population unable to work include persons who were retired for health reasons in 1979 and 1980 , disabled homemakers , and other persons who were disabled for the entire year 1980 but were not retired for health reasons in 1979 , but the Rice et al. estimates do not include the last two categories in the population unable to work .
	manualset3
146918	15	409559	5	NULL	NULL	0	NULL	health reasons	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The differences , which can be resolved , are attributable to two major factors : ( 1 ) NMCUES includes only the civilian noninstitutionalized population , but the other estimates include the institutionalized population and the military ; and ( 2 ) NMCUES indirect cost estimates for the population unable to work include persons who were retired for health reasons in 1979 and 1980 , disabled homemakers , and other persons who were disabled for the entire year 1980 but were not retired for health reasons in 1979 , but the Rice et al. estimates do not include the last two categories in the population unable to work .
	manualset3
146919	16	409559	5	NULL	NULL	0	NULL	1979 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	The differences , which can be resolved , are attributable to two major factors : ( 1 ) NMCUES includes only the civilian noninstitutionalized population , but the other estimates include the institutionalized population and the military ; and ( 2 ) NMCUES indirect cost estimates for the population unable to work include persons who were retired for health reasons in 1979 and 1980 , disabled homemakers , and other persons who were disabled for the entire year 1980 but were not retired for health reasons in 1979 , but the Rice et al. estimates do not include the last two categories in the population unable to work .
	manualset3
146920	17	409559	5	NULL	NULL	0	NULL	Rice et al.	Citation												NULL		0	NULL	NULL	NULL	NULL	NULL	The differences , which can be resolved , are attributable to two major factors : ( 1 ) NMCUES includes only the civilian noninstitutionalized population , but the other estimates include the institutionalized population and the military ; and ( 2 ) NMCUES indirect cost estimates for the population unable to work include persons who were retired for health reasons in 1979 and 1980 , disabled homemakers , and other persons who were disabled for the entire year 1980 but were not retired for health reasons in 1979 , but the Rice et al. estimates do not include the last two categories in the population unable to work .
	manualset3
146921	18	409559	5	NULL	NULL	0	NULL	two categories	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The differences , which can be resolved , are attributable to two major factors : ( 1 ) NMCUES includes only the civilian noninstitutionalized population , but the other estimates include the institutionalized population and the military ; and ( 2 ) NMCUES indirect cost estimates for the population unable to work include persons who were retired for health reasons in 1979 and 1980 , disabled homemakers , and other persons who were disabled for the entire year 1980 but were not retired for health reasons in 1979 , but the Rice et al. estimates do not include the last two categories in the population unable to work .
	manualset3
146922	19	409559	5	NULL	NULL	0	NULL	population 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The differences , which can be resolved , are attributable to two major factors : ( 1 ) NMCUES includes only the civilian noninstitutionalized population , but the other estimates include the institutionalized population and the military ; and ( 2 ) NMCUES indirect cost estimates for the population unable to work include persons who were retired for health reasons in 1979 and 1980 , disabled homemakers , and other persons who were disabled for the entire year 1980 but were not retired for health reasons in 1979 , but the Rice et al. estimates do not include the last two categories in the population unable to work .
	manualset3
146923	1	409560	5	NULL	NULL	0	NULL	differences 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The differences are caused by serum substances ( non-creatinine chromogens ) reacting with picric acid .
	manualset3
146924	2	409560	5	NULL	NULL	0	NULL	serum substances ( non-creatinine chromogens )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The differences are caused by serum substances ( non-creatinine chromogens ) reacting with picric acid .
	manualset3
146925	3	409560	5	NULL	NULL	0	NULL	picric acid	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The differences are caused by serum substances ( non-creatinine chromogens ) reacting with picric acid .
	manualset3
146926	1	409561	5	NULL	NULL	0	NULL	different kinetics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The different kinetics of both MAPK suggest that different signalling cascades were activated .
	manualset3
146927	2	409561	5	NULL	NULL	0	NULL	MAPK 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The different kinetics of both MAPK suggest that different signalling cascades were activated .
	manualset3
146928	3	409561	5	NULL	NULL	0	NULL	signalling cascades 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The different kinetics of both MAPK suggest that different signalling cascades were activated .
	manualset3
146929	1	409562	5	NULL	NULL	0	NULL	ligaments 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The different ligaments of the symphysis pubis in the pregnant and the non-pregnant state .
	manualset3
146930	2	409562	5	NULL	NULL	0	NULL	symphysis pubis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The different ligaments of the symphysis pubis in the pregnant and the non-pregnant state .
	manualset3
146931	3	409562	5	NULL	NULL	0	NULL	pregnant state	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The different ligaments of the symphysis pubis in the pregnant and the non-pregnant state .
	manualset3
146932	4	409562	5	NULL	NULL	0	NULL	non-pregnant state 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The different ligaments of the symphysis pubis in the pregnant and the non-pregnant state .
	manualset3
146933	1	409563	5	NULL	NULL	0	NULL	immunisation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A single immunisation of BALB/c mice with both DS-2 and yeast-cell derived purified HBsAg particles without adjuvants elicited a substantial humoral antibody and class-I restricted cytotoxic T lymphocyte ( CTL ) response .
	manualset3
146934	2	409563	5	NULL	NULL	0	NULL	BALB/c mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A single immunisation of BALB/c mice with both DS-2 and yeast-cell derived purified HBsAg particles without adjuvants elicited a substantial humoral antibody and class-I restricted cytotoxic T lymphocyte ( CTL ) response .
	manualset3
146935	3	409563	5	NULL	NULL	0	NULL	DS-2 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A single immunisation of BALB/c mice with both DS-2 and yeast-cell derived purified HBsAg particles without adjuvants elicited a substantial humoral antibody and class-I restricted cytotoxic T lymphocyte ( CTL ) response .
	manualset3
146936	4	409563	5	NULL	NULL	0	NULL	yeast-cell derived purified HBsAg particles	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A single immunisation of BALB/c mice with both DS-2 and yeast-cell derived purified HBsAg particles without adjuvants elicited a substantial humoral antibody and class-I restricted cytotoxic T lymphocyte ( CTL ) response .
	manualset3
146937	5	409563	5	NULL	NULL	0	NULL	adjuvants 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A single immunisation of BALB/c mice with both DS-2 and yeast-cell derived purified HBsAg particles without adjuvants elicited a substantial humoral antibody and class-I restricted cytotoxic T lymphocyte ( CTL ) response .
	manualset3
146938	6	409563	5	NULL	NULL	0	NULL	substantial humoral antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A single immunisation of BALB/c mice with both DS-2 and yeast-cell derived purified HBsAg particles without adjuvants elicited a substantial humoral antibody and class-I restricted cytotoxic T lymphocyte ( CTL ) response .
	manualset3
146939	7	409563	5	NULL	NULL	0	NULL	class-I restricted cytotoxic T lymphocyte ( CTL ) response 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A single immunisation of BALB/c mice with both DS-2 and yeast-cell derived purified HBsAg particles without adjuvants elicited a substantial humoral antibody and class-I restricted cytotoxic T lymphocyte ( CTL ) response .
	manualset3
146940	1	409564	5	NULL	NULL	0	NULL	different responses 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The different responses of cytosolic and mitochondrial L-alanine : 4 , 5 - dioxovalerate transaminases to hemin supplementation both in vitro and in vivo was demonstrated .
	manualset3
146941	2	409564	5	NULL	NULL	0	NULL	cytosolic L-alanine : 4 , 5 - dioxovalerate transaminase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The different responses of cytosolic and mitochondrial L-alanine : 4 , 5 - dioxovalerate transaminases to hemin supplementation both in vitro and in vivo was demonstrated .
	manualset3
146942	3	409564	5	NULL	NULL	0	NULL	mitochondrial L-alanine : 4 , 5 - dioxovalerate transaminase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The different responses of cytosolic and mitochondrial L-alanine : 4 , 5 - dioxovalerate transaminases to hemin supplementation both in vitro and in vivo was demonstrated .
	manualset3
146943	4	409564	5	NULL	NULL	0	NULL	hemin supplementation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The different responses of cytosolic and mitochondrial L-alanine : 4 , 5 - dioxovalerate transaminases to hemin supplementation both in vitro and in vivo was demonstrated .
	manualset3
146944	1	409565	5	NULL	NULL	0	NULL	different sites of activation 	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The different sites of activation of corticospinal neurons by TMS and TES , as well as the different distribution of D and I responses that they evoke , may both contribute to the differences in the onset latencies of the EMG responses evoked by these methods in human subjects .
	manualset3
146945	2	409565	5	NULL	NULL	0	NULL	corticospinal neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The different sites of activation of corticospinal neurons by TMS and TES , as well as the different distribution of D and I responses that they evoke , may both contribute to the differences in the onset latencies of the EMG responses evoked by these methods in human subjects .
	manualset3
146946	3	409565	5	NULL	NULL	0	NULL	TMS 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The different sites of activation of corticospinal neurons by TMS and TES , as well as the different distribution of D and I responses that they evoke , may both contribute to the differences in the onset latencies of the EMG responses evoked by these methods in human subjects .
	manualset3
146947	4	409565	5	NULL	NULL	0	NULL	TES 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The different sites of activation of corticospinal neurons by TMS and TES , as well as the different distribution of D and I responses that they evoke , may both contribute to the differences in the onset latencies of the EMG responses evoked by these methods in human subjects .
	manualset3
146948	5	409565	5	NULL	NULL	0	NULL	distribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The different sites of activation of corticospinal neurons by TMS and TES , as well as the different distribution of D and I responses that they evoke , may both contribute to the differences in the onset latencies of the EMG responses evoked by these methods in human subjects .
	manualset3
146949	6	409565	5	NULL	NULL	0	NULL	D responses 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The different sites of activation of corticospinal neurons by TMS and TES , as well as the different distribution of D and I responses that they evoke , may both contribute to the differences in the onset latencies of the EMG responses evoked by these methods in human subjects .
	manualset3
146950	7	409565	5	NULL	NULL	0	NULL	I responses 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The different sites of activation of corticospinal neurons by TMS and TES , as well as the different distribution of D and I responses that they evoke , may both contribute to the differences in the onset latencies of the EMG responses evoked by these methods in human subjects .
	manualset3
146951	8	409565	5	NULL	NULL	0	NULL	differences 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The different sites of activation of corticospinal neurons by TMS and TES , as well as the different distribution of D and I responses that they evoke , may both contribute to the differences in the onset latencies of the EMG responses evoked by these methods in human subjects .
	manualset3
146952	9	409565	5	NULL	NULL	0	NULL	onset latencies 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The different sites of activation of corticospinal neurons by TMS and TES , as well as the different distribution of D and I responses that they evoke , may both contribute to the differences in the onset latencies of the EMG responses evoked by these methods in human subjects .
	manualset3
146953	10	409565	5	NULL	NULL	0	NULL	EMG responses 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The different sites of activation of corticospinal neurons by TMS and TES , as well as the different distribution of D and I responses that they evoke , may both contribute to the differences in the onset latencies of the EMG responses evoked by these methods in human subjects .
	manualset3
146954	11	409565	5	NULL	NULL	0	NULL	methods 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The different sites of activation of corticospinal neurons by TMS and TES , as well as the different distribution of D and I responses that they evoke , may both contribute to the differences in the onset latencies of the EMG responses evoked by these methods in human subjects .
	manualset3
146955	12	409565	5	NULL	NULL	0	NULL	human subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The different sites of activation of corticospinal neurons by TMS and TES , as well as the different distribution of D and I responses that they evoke , may both contribute to the differences in the onset latencies of the EMG responses evoked by these methods in human subjects .
	manualset3
146956	1	409566	5	NULL	NULL	0	NULL	volumes 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The different volumes of ropivacaine 0.75 % ( 15 , 20 , and 25 ml ) brought about adequate analgesia in the sacral and lumbar regions in all patients .
	manualset3
146957	2	409566	5	NULL	NULL	0	NULL	ropivacaine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The different volumes of ropivacaine 0.75 % ( 15 , 20 , and 25 ml ) brought about adequate analgesia in the sacral and lumbar regions in all patients .
	manualset3
146958	3	409566	5	NULL	NULL	0	NULL	0.75 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The different volumes of ropivacaine 0.75 % ( 15 , 20 , and 25 ml ) brought about adequate analgesia in the sacral and lumbar regions in all patients .
	manualset3
146959	4	409566	5	NULL	NULL	0	NULL	15 ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The different volumes of ropivacaine 0.75 % ( 15 , 20 , and 25 ml ) brought about adequate analgesia in the sacral and lumbar regions in all patients .
	manualset3
146960	5	409566	5	NULL	NULL	0	NULL	20 ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The different volumes of ropivacaine 0.75 % ( 15 , 20 , and 25 ml ) brought about adequate analgesia in the sacral and lumbar regions in all patients .
	manualset3
146961	6	409566	5	NULL	NULL	0	NULL	25 ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The different volumes of ropivacaine 0.75 % ( 15 , 20 , and 25 ml ) brought about adequate analgesia in the sacral and lumbar regions in all patients .
	manualset3
146962	7	409566	5	NULL	NULL	0	NULL	analgesia 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The different volumes of ropivacaine 0.75 % ( 15 , 20 , and 25 ml ) brought about adequate analgesia in the sacral and lumbar regions in all patients .
	manualset3
146963	8	409566	5	NULL	NULL	0	NULL	sacral regions 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The different volumes of ropivacaine 0.75 % ( 15 , 20 , and 25 ml ) brought about adequate analgesia in the sacral and lumbar regions in all patients .
	manualset3
146964	9	409566	5	NULL	NULL	0	NULL	lumbar regions 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The different volumes of ropivacaine 0.75 % ( 15 , 20 , and 25 ml ) brought about adequate analgesia in the sacral and lumbar regions in all patients .
	manualset3
146965	10	409566	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The different volumes of ropivacaine 0.75 % ( 15 , 20 , and 25 ml ) brought about adequate analgesia in the sacral and lumbar regions in all patients .
	manualset3
146966	1	409567	5	NULL	NULL	0	NULL	differentiated pigment epithelium cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The differentiated pigment epithelium cells also proliferate in this area of the eye .
	manualset3
146967	2	409567	5	NULL	NULL	0	NULL	area of the eye	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The differentiated pigment epithelium cells also proliferate in this area of the eye .
	manualset3
146968	1	409568	5	NULL	NULL	0	NULL	differentiation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The differentiation of U937 monoblastoid cells after human immunodeficiency virus type 1 ( HIV-1 ) infection was studied using the following approaches : reverse transcriptase activity measurement , immunofluorescence labeling , and electron microscopy .
	manualset3
146969	2	409568	5	NULL	NULL	0	NULL	U937 monoblastoid cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The differentiation of U937 monoblastoid cells after human immunodeficiency virus type 1 ( HIV-1 ) infection was studied using the following approaches : reverse transcriptase activity measurement , immunofluorescence labeling , and electron microscopy .
	manualset3
146970	3	409568	5	NULL	NULL	0	NULL	human immunodeficiency virus type 1 ( HIV-1 ) infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The differentiation of U937 monoblastoid cells after human immunodeficiency virus type 1 ( HIV-1 ) infection was studied using the following approaches : reverse transcriptase activity measurement , immunofluorescence labeling , and electron microscopy .
	manualset3
146971	4	409568	5	NULL	NULL	0	NULL	approaches 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The differentiation of U937 monoblastoid cells after human immunodeficiency virus type 1 ( HIV-1 ) infection was studied using the following approaches : reverse transcriptase activity measurement , immunofluorescence labeling , and electron microscopy .
	manualset3
146972	5	409568	5	NULL	NULL	0	NULL	reverse transcriptase activity measurement	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The differentiation of U937 monoblastoid cells after human immunodeficiency virus type 1 ( HIV-1 ) infection was studied using the following approaches : reverse transcriptase activity measurement , immunofluorescence labeling , and electron microscopy .
	manualset3
146973	6	409568	5	NULL	NULL	0	NULL	immunofluorescence labeling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The differentiation of U937 monoblastoid cells after human immunodeficiency virus type 1 ( HIV-1 ) infection was studied using the following approaches : reverse transcriptase activity measurement , immunofluorescence labeling , and electron microscopy .
	manualset3
146974	7	409568	5	NULL	NULL	0	NULL	electron microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The differentiation of U937 monoblastoid cells after human immunodeficiency virus type 1 ( HIV-1 ) infection was studied using the following approaches : reverse transcriptase activity measurement , immunofluorescence labeling , and electron microscopy .
	manualset3
146975	1	409569	5	NULL	NULL	0	NULL	differentiation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The differentiation of cells was dependent on the concentration of gangliosides and was accompanied by inhibition of cell growth .
	manualset3
146976	2	409569	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The differentiation of cells was dependent on the concentration of gangliosides and was accompanied by inhibition of cell growth .
	manualset3
146977	3	409569	5	NULL	NULL	0	NULL	concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The differentiation of cells was dependent on the concentration of gangliosides and was accompanied by inhibition of cell growth .
	manualset3
146978	4	409569	5	NULL	NULL	0	NULL	gangliosides 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The differentiation of cells was dependent on the concentration of gangliosides and was accompanied by inhibition of cell growth .
	manualset3
146979	5	409569	5	NULL	NULL	0	NULL	inhibition of cell growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The differentiation of cells was dependent on the concentration of gangliosides and was accompanied by inhibition of cell growth .
	manualset3
146980	1	409570	5	NULL	NULL	0	NULL	vitamin B12 binding capacities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The differing vitamin B12 binding capacities of neutral and acidified material was utilized to fractionate the unsaturated vitamin B12-binding proteins of serum and plasma .
	manualset3
146981	2	409570	5	NULL	NULL	NULL	NULL	neutral material 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The differing vitamin B12 binding capacities of neutral and acidified material was utilized to fractionate the unsaturated vitamin B12-binding proteins of serum and plasma .
	manualset3
146982	3	409570	5	NULL	NULL	NULL	NULL	acidified material 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The differing vitamin B12 binding capacities of neutral and acidified material was utilized to fractionate the unsaturated vitamin B12-binding proteins of serum and plasma .
	manualset3
146983	4	409570	5	NULL	NULL	0	NULL	unsaturated vitamin B12-binding proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The differing vitamin B12 binding capacities of neutral and acidified material was utilized to fractionate the unsaturated vitamin B12-binding proteins of serum and plasma .
	manualset3
146984	5	409570	5	NULL	NULL	0	NULL	serum 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The differing vitamin B12 binding capacities of neutral and acidified material was utilized to fractionate the unsaturated vitamin B12-binding proteins of serum and plasma .
	manualset3
146985	6	409570	5	NULL	NULL	0	NULL	plasma 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The differing vitamin B12 binding capacities of neutral and acidified material was utilized to fractionate the unsaturated vitamin B12-binding proteins of serum and plasma .
	manualset3
146986	1	409571	5	NULL	NULL	0	NULL	completeness 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The difficulty of assessing the completeness of a cervical cone and of evaluating a postconization smear is confirmed .
	manualset3
146987	2	409571	5	NULL	NULL	0	NULL	cervical cone 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The difficulty of assessing the completeness of a cervical cone and of evaluating a postconization smear is confirmed .
	manualset3
146988	3	409571	5	NULL	NULL	0	NULL	postconization smear	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The difficulty of assessing the completeness of a cervical cone and of evaluating a postconization smear is confirmed .
	manualset3
146989	1	409572	5	NULL	NULL	0	NULL	single local intramuscular injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A single local intramuscular injection of RoY peptide to the operated limb , significantly restored blood perfusion and alleviated hind limb ischemia as determined by a laser Doppler imager .
	manualset3
146990	2	409572	5	NULL	NULL	0	NULL	RoY peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	A single local intramuscular injection of RoY peptide to the operated limb , significantly restored blood perfusion and alleviated hind limb ischemia as determined by a laser Doppler imager .
	manualset3
146991	3	409572	5	NULL	NULL	0	NULL	operated limb	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A single local intramuscular injection of RoY peptide to the operated limb , significantly restored blood perfusion and alleviated hind limb ischemia as determined by a laser Doppler imager .
	manualset3
146992	4	409572	5	NULL	NULL	0	NULL	blood perfusion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A single local intramuscular injection of RoY peptide to the operated limb , significantly restored blood perfusion and alleviated hind limb ischemia as determined by a laser Doppler imager .
	manualset3
146993	5	409572	5	NULL	NULL	0	NULL	alleviated hind limb ischemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A single local intramuscular injection of RoY peptide to the operated limb , significantly restored blood perfusion and alleviated hind limb ischemia as determined by a laser Doppler imager .
	manualset3
146994	6	409572	5	NULL	NULL	0	NULL	laser Doppler imager	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A single local intramuscular injection of RoY peptide to the operated limb , significantly restored blood perfusion and alleviated hind limb ischemia as determined by a laser Doppler imager .
	manualset3
146995	1	409573	5	NULL	NULL	0	NULL	diffusion 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The diffusion of plastoquinol in the chloroplast thylakoid membrane is modelled using Monte Carlo techniques .
	manualset3
146996	2	409573	5	NULL	NULL	0	NULL	plastoquinol 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The diffusion of plastoquinol in the chloroplast thylakoid membrane is modelled using Monte Carlo techniques .
	manualset3
146997	3	409573	5	NULL	NULL	0	NULL	chloroplast thylakoid membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The diffusion of plastoquinol in the chloroplast thylakoid membrane is modelled using Monte Carlo techniques .
	manualset3
146998	4	409573	5	NULL	NULL	0	NULL	Monte Carlo techniques	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The diffusion of plastoquinol in the chloroplast thylakoid membrane is modelled using Monte Carlo techniques .
	manualset3
146999	1	409574	5	NULL	NULL	0	NULL	digestibility values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The digestibility values for wheat acquired with the difference method for ration 1 were 85.7 % for crude protein , 57.0 % for crude fat and 89.8 % for N-free extractives ; energy concentration was 766 EFUhens .
	manualset3
147000	2	409574	5	NULL	NULL	0	NULL	wheat 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The digestibility values for wheat acquired with the difference method for ration 1 were 85.7 % for crude protein , 57.0 % for crude fat and 89.8 % for N-free extractives ; energy concentration was 766 EFUhens .
	manualset3
147001	3	409574	5	NULL	NULL	0	NULL	difference method 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The digestibility values for wheat acquired with the difference method for ration 1 were 85.7 % for crude protein , 57.0 % for crude fat and 89.8 % for N-free extractives ; energy concentration was 766 EFUhens .
	manualset3
147002	4	409574	5	NULL	NULL	0	NULL	ration 1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The digestibility values for wheat acquired with the difference method for ration 1 were 85.7 % for crude protein , 57.0 % for crude fat and 89.8 % for N-free extractives ; energy concentration was 766 EFUhens .
	manualset3
147003	5	409574	5	NULL	NULL	0	NULL	85.7 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The digestibility values for wheat acquired with the difference method for ration 1 were 85.7 % for crude protein , 57.0 % for crude fat and 89.8 % for N-free extractives ; energy concentration was 766 EFUhens .
	manualset3
147004	6	409574	5	NULL	NULL	0	NULL	crude protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The digestibility values for wheat acquired with the difference method for ration 1 were 85.7 % for crude protein , 57.0 % for crude fat and 89.8 % for N-free extractives ; energy concentration was 766 EFUhens .
	manualset3
147005	7	409574	5	NULL	NULL	0	NULL	57.0 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The digestibility values for wheat acquired with the difference method for ration 1 were 85.7 % for crude protein , 57.0 % for crude fat and 89.8 % for N-free extractives ; energy concentration was 766 EFUhens .
	manualset3
147006	8	409574	5	NULL	NULL	0	NULL	crude fat	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The digestibility values for wheat acquired with the difference method for ration 1 were 85.7 % for crude protein , 57.0 % for crude fat and 89.8 % for N-free extractives ; energy concentration was 766 EFUhens .
	manualset3
147007	9	409574	5	NULL	NULL	0	NULL	 89.8 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The digestibility values for wheat acquired with the difference method for ration 1 were 85.7 % for crude protein , 57.0 % for crude fat and 89.8 % for N-free extractives ; energy concentration was 766 EFUhens .
	manualset3
147008	10	409574	5	NULL	NULL	0	NULL	N-free extractives	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The digestibility values for wheat acquired with the difference method for ration 1 were 85.7 % for crude protein , 57.0 % for crude fat and 89.8 % for N-free extractives ; energy concentration was 766 EFUhens .
	manualset3
147009	11	409574	5	NULL	NULL	0	NULL	energy concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The digestibility values for wheat acquired with the difference method for ration 1 were 85.7 % for crude protein , 57.0 % for crude fat and 89.8 % for N-free extractives ; energy concentration was 766 EFUhens .
	manualset3
147010	12	409574	5	NULL	NULL	0	NULL	766 EFUhens	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The digestibility values for wheat acquired with the difference method for ration 1 were 85.7 % for crude protein , 57.0 % for crude fat and 89.8 % for N-free extractives ; energy concentration was 766 EFUhens .
	manualset3
147011	1	409575	5	NULL	NULL	0	NULL	dihedral angles 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The dihedral angles between the carboxyl-ate groups and the adjacent benzene rings are 10.89 ( 16 ) and 8.4 ( 2 ) , while the benzene rings are oriented at a dihedral angle of 6.09 ( 13 ) .
	manualset3
147012	2	409575	5	NULL	NULL	0	NULL	carboxyl-ate groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The dihedral angles between the carboxyl-ate groups and the adjacent benzene rings are 10.89 ( 16 ) and 8.4 ( 2 ) , while the benzene rings are oriented at a dihedral angle of 6.09 ( 13 ) .
	manualset3
147013	3	409575	5	NULL	NULL	0	NULL	adjacent benzene rings	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The dihedral angles between the carboxyl-ate groups and the adjacent benzene rings are 10.89 ( 16 ) and 8.4 ( 2 ) , while the benzene rings are oriented at a dihedral angle of 6.09 ( 13 ) .
	manualset3
147014	4	409575	5	NULL	NULL	0	NULL	10.89 ( 16 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The dihedral angles between the carboxyl-ate groups and the adjacent benzene rings are 10.89 ( 16 ) and 8.4 ( 2 ) , while the benzene rings are oriented at a dihedral angle of 6.09 ( 13 ) .
	manualset3
147015	5	409575	5	NULL	NULL	0	NULL	8.4 ( 2 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The dihedral angles between the carboxyl-ate groups and the adjacent benzene rings are 10.89 ( 16 ) and 8.4 ( 2 ) , while the benzene rings are oriented at a dihedral angle of 6.09 ( 13 ) .
	manualset3
147016	6	409575	5	NULL	NULL	0	NULL	benzene rings	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The dihedral angles between the carboxyl-ate groups and the adjacent benzene rings are 10.89 ( 16 ) and 8.4 ( 2 ) , while the benzene rings are oriented at a dihedral angle of 6.09 ( 13 ) .
	manualset3
147017	7	409575	5	NULL	NULL	0	NULL	dihedral angle	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The dihedral angles between the carboxyl-ate groups and the adjacent benzene rings are 10.89 ( 16 ) and 8.4 ( 2 ) , while the benzene rings are oriented at a dihedral angle of 6.09 ( 13 ) .
	manualset3
147018	8	409575	5	NULL	NULL	0	NULL	6.09 ( 13 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The dihedral angles between the carboxyl-ate groups and the adjacent benzene rings are 10.89 ( 16 ) and 8.4 ( 2 ) , while the benzene rings are oriented at a dihedral angle of 6.09 ( 13 ) .
	manualset3
147019	1	409576	5	NULL	NULL	0	NULL	dihydrofolate reductase-deficient Chinese hamster ovary cell line , DXB11-CHO	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The dihydrofolate reductase-deficient Chinese hamster ovary cell line , DXB11-CHO , commonly used as a host cell for the production of recombinant proteins requires 7.5 % serum-supplementation for optimal growth .
	manualset3
147020	2	409576	5	NULL	NULL	0	NULL	host cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The dihydrofolate reductase-deficient Chinese hamster ovary cell line , DXB11-CHO , commonly used as a host cell for the production of recombinant proteins requires 7.5 % serum-supplementation for optimal growth .
	manualset3
147021	3	409576	5	NULL	NULL	0	NULL	production 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dihydrofolate reductase-deficient Chinese hamster ovary cell line , DXB11-CHO , commonly used as a host cell for the production of recombinant proteins requires 7.5 % serum-supplementation for optimal growth .
	manualset3
147022	4	409576	5	NULL	NULL	0	NULL	recombinant proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The dihydrofolate reductase-deficient Chinese hamster ovary cell line , DXB11-CHO , commonly used as a host cell for the production of recombinant proteins requires 7.5 % serum-supplementation for optimal growth .
	manualset3
147023	5	409576	5	NULL	NULL	NULL	NULL	 7.5 % 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The dihydrofolate reductase-deficient Chinese hamster ovary cell line , DXB11-CHO , commonly used as a host cell for the production of recombinant proteins requires 7.5 % serum-supplementation for optimal growth .
	manualset3
147024	6	409576	5	NULL	NULL	0	NULL	serum-supplementation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dihydrofolate reductase-deficient Chinese hamster ovary cell line , DXB11-CHO , commonly used as a host cell for the production of recombinant proteins requires 7.5 % serum-supplementation for optimal growth .
	manualset3
147025	7	409576	5	NULL	NULL	0	NULL	optimal growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The dihydrofolate reductase-deficient Chinese hamster ovary cell line , DXB11-CHO , commonly used as a host cell for the production of recombinant proteins requires 7.5 % serum-supplementation for optimal growth .
	manualset3
147026	1	409577	5	NULL	NULL	0	NULL	dilatation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dilatation has no long-term effect in malignant stenoses so it was used just for diagnosis or in rare inoperable cases for the preparation of prosthesis implantation .
	manualset3
147027	2	409577	5	NULL	NULL	0	NULL	long-term effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dilatation has no long-term effect in malignant stenoses so it was used just for diagnosis or in rare inoperable cases for the preparation of prosthesis implantation .
	manualset3
147028	3	409577	5	NULL	NULL	0	NULL	malignant stenoses 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The dilatation has no long-term effect in malignant stenoses so it was used just for diagnosis or in rare inoperable cases for the preparation of prosthesis implantation .
	manualset3
147029	4	409577	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The dilatation has no long-term effect in malignant stenoses so it was used just for diagnosis or in rare inoperable cases for the preparation of prosthesis implantation .
	manualset3
147030	5	409577	5	NULL	NULL	0	NULL	rare inoperable cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The dilatation has no long-term effect in malignant stenoses so it was used just for diagnosis or in rare inoperable cases for the preparation of prosthesis implantation .
	manualset3
147031	6	409577	5	NULL	NULL	0	NULL	preparation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The dilatation has no long-term effect in malignant stenoses so it was used just for diagnosis or in rare inoperable cases for the preparation of prosthesis implantation .
	manualset3
147032	7	409577	5	NULL	NULL	0	NULL	prosthesis implantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The dilatation has no long-term effect in malignant stenoses so it was used just for diagnosis or in rare inoperable cases for the preparation of prosthesis implantation .
	manualset3
147033	1	409578	5	NULL	NULL	0	NULL	single species , sweet pea ( Lathyrus odoratus ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A single species , sweet pea ( Lathyrus odoratus ) , contains a second PII transcript which is 0.2 kb larger than the approximately 1.2 kb transcript found in all species .
	manualset3
147034	2	409578	5	NULL	NULL	0	NULL	second PII transcript	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A single species , sweet pea ( Lathyrus odoratus ) , contains a second PII transcript which is 0.2 kb larger than the approximately 1.2 kb transcript found in all species .
	manualset3
147035	3	409578	5	NULL	NULL	0	NULL	0.2 kb	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A single species , sweet pea ( Lathyrus odoratus ) , contains a second PII transcript which is 0.2 kb larger than the approximately 1.2 kb transcript found in all species .
	manualset3
147036	4	409578	5	NULL	NULL	0	NULL	 1.2 kb transcript	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A single species , sweet pea ( Lathyrus odoratus ) , contains a second PII transcript which is 0.2 kb larger than the approximately 1.2 kb transcript found in all species .
	manualset3
147037	5	409578	5	NULL	NULL	0	NULL	species 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A single species , sweet pea ( Lathyrus odoratus ) , contains a second PII transcript which is 0.2 kb larger than the approximately 1.2 kb transcript found in all species .
	manualset3
147038	1	409579	5	NULL	NULL	0	NULL	direct effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The direct effects of prostaglandin E-1 ( PGE-1 ) and F-2 alpha ( PGF-2alpha ) on isolated mouse oocytes were examined in a microtube culture method .
	manualset3
147039	2	409579	5	NULL	NULL	0	NULL	prostaglandin E-1 ( PGE-1 )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The direct effects of prostaglandin E-1 ( PGE-1 ) and F-2 alpha ( PGF-2alpha ) on isolated mouse oocytes were examined in a microtube culture method .
	manualset3
147040	3	409579	5	NULL	NULL	0	NULL	F-2 alpha ( PGF-2alpha )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The direct effects of prostaglandin E-1 ( PGE-1 ) and F-2 alpha ( PGF-2alpha ) on isolated mouse oocytes were examined in a microtube culture method .
	manualset3
147041	4	409579	5	NULL	NULL	0	NULL	isolated mouse oocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The direct effects of prostaglandin E-1 ( PGE-1 ) and F-2 alpha ( PGF-2alpha ) on isolated mouse oocytes were examined in a microtube culture method .
	manualset3
147042	5	409579	5	NULL	NULL	0	NULL	microtube culture method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The direct effects of prostaglandin E-1 ( PGE-1 ) and F-2 alpha ( PGF-2alpha ) on isolated mouse oocytes were examined in a microtube culture method .
	manualset3
147043	1	409580	5	NULL	NULL	0	NULL	direct involvement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The direct involvement of Gq/11/phospholipase C signaling and the ERK-1 / 2 and JNK pathways together with receptor phosphorylation in the anti-apoptotic response were eliminated .
	manualset3
147044	2	409580	5	NULL	NULL	0	NULL	Gq/11/phospholipase C signaling 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The direct involvement of Gq/11/phospholipase C signaling and the ERK-1 / 2 and JNK pathways together with receptor phosphorylation in the anti-apoptotic response were eliminated .
	manualset3
147045	3	409580	5	NULL	NULL	0	NULL	ERK-1 / 2 pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The direct involvement of Gq/11/phospholipase C signaling and the ERK-1 / 2 and JNK pathways together with receptor phosphorylation in the anti-apoptotic response were eliminated .
	manualset3
147046	4	409580	5	NULL	NULL	0	NULL	JNK pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The direct involvement of Gq/11/phospholipase C signaling and the ERK-1 / 2 and JNK pathways together with receptor phosphorylation in the anti-apoptotic response were eliminated .
	manualset3
147047	5	409580	5	NULL	NULL	0	NULL	receptor phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The direct involvement of Gq/11/phospholipase C signaling and the ERK-1 / 2 and JNK pathways together with receptor phosphorylation in the anti-apoptotic response were eliminated .
	manualset3
147048	6	409580	5	NULL	NULL	0	NULL	anti-apoptotic response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The direct involvement of Gq/11/phospholipase C signaling and the ERK-1 / 2 and JNK pathways together with receptor phosphorylation in the anti-apoptotic response were eliminated .
	manualset3
147049	1	409581	5	NULL	NULL	0	NULL	direct observation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The direct observation of drug release from carbon nanotube vehicles in living cells is realized through a unique two-dye labeling approach .
	manualset3
147050	2	409581	5	NULL	NULL	0	NULL	drug release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The direct observation of drug release from carbon nanotube vehicles in living cells is realized through a unique two-dye labeling approach .
	manualset3
147051	3	409581	5	NULL	NULL	0	NULL	carbon nanotube vehicles 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The direct observation of drug release from carbon nanotube vehicles in living cells is realized through a unique two-dye labeling approach .
	manualset3
147052	4	409581	5	NULL	NULL	0	NULL	living cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The direct observation of drug release from carbon nanotube vehicles in living cells is realized through a unique two-dye labeling approach .
	manualset3
147053	5	409581	5	NULL	NULL	0	NULL	two-dye labeling approach 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The direct observation of drug release from carbon nanotube vehicles in living cells is realized through a unique two-dye labeling approach .
	manualset3
147054	1	409582	5	NULL	NULL	0	NULL	direction 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The direction of translocation has been determined using a helicase assay that directly measures the ability of helicase II to catalyze the displacement of a labeled DNA fragment from one end of a single-stranded linear DNA molecule .
	manualset3
147055	2	409582	5	NULL	NULL	0	NULL	translocation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The direction of translocation has been determined using a helicase assay that directly measures the ability of helicase II to catalyze the displacement of a labeled DNA fragment from one end of a single-stranded linear DNA molecule .
	manualset3
147056	3	409582	5	NULL	NULL	0	NULL	helicase assay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The direction of translocation has been determined using a helicase assay that directly measures the ability of helicase II to catalyze the displacement of a labeled DNA fragment from one end of a single-stranded linear DNA molecule .
	manualset3
147057	4	409582	5	NULL	NULL	0	NULL	ability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The direction of translocation has been determined using a helicase assay that directly measures the ability of helicase II to catalyze the displacement of a labeled DNA fragment from one end of a single-stranded linear DNA molecule .
	manualset3
147058	5	409582	5	NULL	NULL	0	NULL	helicase II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The direction of translocation has been determined using a helicase assay that directly measures the ability of helicase II to catalyze the displacement of a labeled DNA fragment from one end of a single-stranded linear DNA molecule .
	manualset3
147059	6	409582	5	NULL	NULL	0	NULL	displacement 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The direction of translocation has been determined using a helicase assay that directly measures the ability of helicase II to catalyze the displacement of a labeled DNA fragment from one end of a single-stranded linear DNA molecule .
	manualset3
147060	7	409582	5	NULL	NULL	0	NULL	labeled DNA fragment 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The direction of translocation has been determined using a helicase assay that directly measures the ability of helicase II to catalyze the displacement of a labeled DNA fragment from one end of a single-stranded linear DNA molecule .
	manualset3
147061	8	409582	5	NULL	NULL	0	NULL	single-stranded linear DNA molecule	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The direction of translocation has been determined using a helicase assay that directly measures the ability of helicase II to catalyze the displacement of a labeled DNA fragment from one end of a single-stranded linear DNA molecule .
	manualset3
147062	1	409583	5	NULL	NULL	0	NULL	disability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The disability resulting from uni-or bilateral loss of vestibular function was assessed by exposing subjects , in darkness , to random rotational displacements on a motorized chair away from a `` center '' position and requiring them to rotate themselves back to center using a `` joystick '' control .
	manualset3
147063	2	409583	5	NULL	NULL	0	NULL	uni-or bilateral loss 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The disability resulting from uni-or bilateral loss of vestibular function was assessed by exposing subjects , in darkness , to random rotational displacements on a motorized chair away from a `` center '' position and requiring them to rotate themselves back to center using a `` joystick '' control .
	manualset3
147064	3	409583	5	NULL	NULL	0	NULL	vestibular function 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The disability resulting from uni-or bilateral loss of vestibular function was assessed by exposing subjects , in darkness , to random rotational displacements on a motorized chair away from a `` center '' position and requiring them to rotate themselves back to center using a `` joystick '' control .
	manualset3
147065	4	409583	5	NULL	NULL	0	NULL	subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The disability resulting from uni-or bilateral loss of vestibular function was assessed by exposing subjects , in darkness , to random rotational displacements on a motorized chair away from a `` center '' position and requiring them to rotate themselves back to center using a `` joystick '' control .
	manualset3
147066	5	409583	5	NULL	NULL	0	NULL	darkness 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The disability resulting from uni-or bilateral loss of vestibular function was assessed by exposing subjects , in darkness , to random rotational displacements on a motorized chair away from a `` center '' position and requiring them to rotate themselves back to center using a `` joystick '' control .
	manualset3
147067	6	409583	5	NULL	NULL	0	NULL	random rotational displacements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The disability resulting from uni-or bilateral loss of vestibular function was assessed by exposing subjects , in darkness , to random rotational displacements on a motorized chair away from a `` center '' position and requiring them to rotate themselves back to center using a `` joystick '' control .
	manualset3
147068	7	409583	5	NULL	NULL	0	NULL	motorized chair	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The disability resulting from uni-or bilateral loss of vestibular function was assessed by exposing subjects , in darkness , to random rotational displacements on a motorized chair away from a `` center '' position and requiring them to rotate themselves back to center using a `` joystick '' control .
	manualset3
147069	8	409583	5	NULL	NULL	0	NULL	`` center '' position 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The disability resulting from uni-or bilateral loss of vestibular function was assessed by exposing subjects , in darkness , to random rotational displacements on a motorized chair away from a `` center '' position and requiring them to rotate themselves back to center using a `` joystick '' control .
	manualset3
147070	9	409583	5	NULL	NULL	0	NULL	center 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The disability resulting from uni-or bilateral loss of vestibular function was assessed by exposing subjects , in darkness , to random rotational displacements on a motorized chair away from a `` center '' position and requiring them to rotate themselves back to center using a `` joystick '' control .
	manualset3
147071	10	409583	5	NULL	NULL	0	NULL	`` joystick '' control	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The disability resulting from uni-or bilateral loss of vestibular function was assessed by exposing subjects , in darkness , to random rotational displacements on a motorized chair away from a `` center '' position and requiring them to rotate themselves back to center using a `` joystick '' control .
	manualset3
147072	1	409584	5	NULL	NULL	0	NULL	discharge of nerve impulses	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The discharge of nerve impulses from ommatidia at various distances from one another may be described quantitatively by a set of simultaneous linear equations which express the excitatory effects of the illumination on each ommatidium and the inhibitory interactions between each ommatidium and its neighbors .
	manualset3
147073	2	409584	5	NULL	NULL	0	NULL	ommatidia 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The discharge of nerve impulses from ommatidia at various distances from one another may be described quantitatively by a set of simultaneous linear equations which express the excitatory effects of the illumination on each ommatidium and the inhibitory interactions between each ommatidium and its neighbors .
	manualset3
147074	3	409584	5	NULL	NULL	0	NULL	distances 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The discharge of nerve impulses from ommatidia at various distances from one another may be described quantitatively by a set of simultaneous linear equations which express the excitatory effects of the illumination on each ommatidium and the inhibitory interactions between each ommatidium and its neighbors .
	manualset3
147075	4	409584	5	NULL	NULL	0	NULL	set 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The discharge of nerve impulses from ommatidia at various distances from one another may be described quantitatively by a set of simultaneous linear equations which express the excitatory effects of the illumination on each ommatidium and the inhibitory interactions between each ommatidium and its neighbors .
	manualset3
147076	5	409584	5	NULL	NULL	0	NULL	simultaneous linear equations 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The discharge of nerve impulses from ommatidia at various distances from one another may be described quantitatively by a set of simultaneous linear equations which express the excitatory effects of the illumination on each ommatidium and the inhibitory interactions between each ommatidium and its neighbors .
	manualset3
147077	6	409584	5	NULL	NULL	0	NULL	excitatory effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The discharge of nerve impulses from ommatidia at various distances from one another may be described quantitatively by a set of simultaneous linear equations which express the excitatory effects of the illumination on each ommatidium and the inhibitory interactions between each ommatidium and its neighbors .
	manualset3
147078	7	409584	5	NULL	NULL	0	NULL	illumination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The discharge of nerve impulses from ommatidia at various distances from one another may be described quantitatively by a set of simultaneous linear equations which express the excitatory effects of the illumination on each ommatidium and the inhibitory interactions between each ommatidium and its neighbors .
	manualset3
147079	8	409584	5	NULL	NULL	0	NULL	ommatidium 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The discharge of nerve impulses from ommatidia at various distances from one another may be described quantitatively by a set of simultaneous linear equations which express the excitatory effects of the illumination on each ommatidium and the inhibitory interactions between each ommatidium and its neighbors .
	manualset3
147080	9	409584	5	NULL	NULL	0	NULL	inhibitory interactions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The discharge of nerve impulses from ommatidia at various distances from one another may be described quantitatively by a set of simultaneous linear equations which express the excitatory effects of the illumination on each ommatidium and the inhibitory interactions between each ommatidium and its neighbors .
	manualset3
147081	10	409584	5	NULL	NULL	0	NULL	ommatidium 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The discharge of nerve impulses from ommatidia at various distances from one another may be described quantitatively by a set of simultaneous linear equations which express the excitatory effects of the illumination on each ommatidium and the inhibitory interactions between each ommatidium and its neighbors .
	manualset3
147082	11	409584	5	NULL	NULL	0	NULL	neighbors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The discharge of nerve impulses from ommatidia at various distances from one another may be described quantitatively by a set of simultaneous linear equations which express the excitatory effects of the illumination on each ommatidium and the inhibitory interactions between each ommatidium and its neighbors .
	manualset3
147083	1	409585	5	NULL	NULL	0	NULL	discomfort 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The discomfort due to the edema in the soles of both feet remained even after steroid therapy .
	manualset3
147084	2	409585	5	NULL	NULL	0	NULL	edema 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The discomfort due to the edema in the soles of both feet remained even after steroid therapy .
	manualset3
147086	3	409585	5	NULL	NULL	NULL	NULL	soles of both feet	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The discomfort due to the edema in the soles of both feet remained even after steroid therapy .
	manualset3
147087	4	409585	5	NULL	NULL	0	NULL	steroid therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The discomfort due to the edema in the soles of both feet remained even after steroid therapy .
	manualset3
147088	1	409586	5	NULL	NULL	0	NULL	discordance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The discordance between the ( amputated ) hand motor command and the feedback from above-elbow muscles might partially explain why subjects exhibiting large EMG modulation during phantom hand movement have more phantom limb pain .
	manualset3
147089	2	409586	5	NULL	NULL	0	NULL	( amputated ) hand motor command	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The discordance between the ( amputated ) hand motor command and the feedback from above-elbow muscles might partially explain why subjects exhibiting large EMG modulation during phantom hand movement have more phantom limb pain .
	manualset3
147090	3	409586	5	NULL	NULL	0	NULL	feedback 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The discordance between the ( amputated ) hand motor command and the feedback from above-elbow muscles might partially explain why subjects exhibiting large EMG modulation during phantom hand movement have more phantom limb pain .
	manualset3
147091	4	409586	5	NULL	NULL	0	NULL	above-elbow muscles	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The discordance between the ( amputated ) hand motor command and the feedback from above-elbow muscles might partially explain why subjects exhibiting large EMG modulation during phantom hand movement have more phantom limb pain .
	manualset3
147092	5	409586	5	NULL	NULL	0	NULL	subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The discordance between the ( amputated ) hand motor command and the feedback from above-elbow muscles might partially explain why subjects exhibiting large EMG modulation during phantom hand movement have more phantom limb pain .
	manualset3
147093	6	409586	5	NULL	NULL	0	NULL	large EMG modulation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The discordance between the ( amputated ) hand motor command and the feedback from above-elbow muscles might partially explain why subjects exhibiting large EMG modulation during phantom hand movement have more phantom limb pain .
	manualset3
147094	7	409586	5	NULL	NULL	0	NULL	phantom hand movement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The discordance between the ( amputated ) hand motor command and the feedback from above-elbow muscles might partially explain why subjects exhibiting large EMG modulation during phantom hand movement have more phantom limb pain .
	manualset3
147095	8	409586	5	NULL	NULL	0	NULL	phantom limb pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The discordance between the ( amputated ) hand motor command and the feedback from above-elbow muscles might partially explain why subjects exhibiting large EMG modulation during phantom hand movement have more phantom limb pain .
	manualset3
147096	1	409587	5	NULL	NULL	0	NULL	discovery 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The discovery of atoxyl in 1905 provided doctors with their first therapeutic weapon and , in 1910 , the first action of vector control was undertaken with success in the Island of Principe .
	manualset3
147097	2	409587	5	NULL	NULL	0	NULL	atoxyl 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The discovery of atoxyl in 1905 provided doctors with their first therapeutic weapon and , in 1910 , the first action of vector control was undertaken with success in the Island of Principe .
	manualset3
147098	3	409587	5	NULL	NULL	0	NULL	1905 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	The discovery of atoxyl in 1905 provided doctors with their first therapeutic weapon and , in 1910 , the first action of vector control was undertaken with success in the Island of Principe .
	manualset3
147099	4	409587	5	NULL	NULL	0	NULL	doctors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The discovery of atoxyl in 1905 provided doctors with their first therapeutic weapon and , in 1910 , the first action of vector control was undertaken with success in the Island of Principe .
	manualset3
147100	5	409587	5	NULL	NULL	0	NULL	first therapeutic weapon	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The discovery of atoxyl in 1905 provided doctors with their first therapeutic weapon and , in 1910 , the first action of vector control was undertaken with success in the Island of Principe .
	manualset3
147101	6	409587	5	NULL	NULL	0	NULL	1910 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	The discovery of atoxyl in 1905 provided doctors with their first therapeutic weapon and , in 1910 , the first action of vector control was undertaken with success in the Island of Principe .
	manualset3
147102	7	409587	5	NULL	NULL	0	NULL	first action	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The discovery of atoxyl in 1905 provided doctors with their first therapeutic weapon and , in 1910 , the first action of vector control was undertaken with success in the Island of Principe .
	manualset3
147103	8	409587	5	NULL	NULL	0	NULL	vector control	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The discovery of atoxyl in 1905 provided doctors with their first therapeutic weapon and , in 1910 , the first action of vector control was undertaken with success in the Island of Principe .
	manualset3
147104	9	409587	5	NULL	NULL	0	NULL	success 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The discovery of atoxyl in 1905 provided doctors with their first therapeutic weapon and , in 1910 , the first action of vector control was undertaken with success in the Island of Principe .
	manualset3
147105	10	409587	5	NULL	NULL	0	NULL	Island of Principe	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The discovery of atoxyl in 1905 provided doctors with their first therapeutic weapon and , in 1910 , the first action of vector control was undertaken with success in the Island of Principe .
	manualset3
147106	1	409588	5	NULL	NULL	0	NULL	discovery 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The discovery of multiple transcripts of laminin receptor genes suggests that there is a strong selective pressure to maintain laminin receptor expression in murine cells .
	manualset3
147107	2	409588	5	NULL	NULL	0	NULL	multiple transcripts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The discovery of multiple transcripts of laminin receptor genes suggests that there is a strong selective pressure to maintain laminin receptor expression in murine cells .
	manualset3
147108	3	409588	5	NULL	NULL	0	NULL	laminin receptor genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The discovery of multiple transcripts of laminin receptor genes suggests that there is a strong selective pressure to maintain laminin receptor expression in murine cells .
	manualset3
147109	4	409588	5	NULL	NULL	0	NULL	strong selective pressure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The discovery of multiple transcripts of laminin receptor genes suggests that there is a strong selective pressure to maintain laminin receptor expression in murine cells .
	manualset3
147110	5	409588	5	NULL	NULL	0	NULL	laminin receptor expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The discovery of multiple transcripts of laminin receptor genes suggests that there is a strong selective pressure to maintain laminin receptor expression in murine cells .
	manualset3
147111	6	409588	5	NULL	NULL	0	NULL	murine cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The discovery of multiple transcripts of laminin receptor genes suggests that there is a strong selective pressure to maintain laminin receptor expression in murine cells .
	manualset3
147112	1	409589	5	NULL	NULL	0	NULL	discrepancy 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The discrepancy is likely due to in-medium effects distorting the L-shell electron orbitals .
	manualset3
147113	2	409589	5	NULL	NULL	0	NULL	in-medium effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The discrepancy is likely due to in-medium effects distorting the L-shell electron orbitals .
	manualset3
147114	3	409589	5	NULL	NULL	0	NULL	 L-shell electron orbitals	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The discrepancy is likely due to in-medium effects distorting the L-shell electron orbitals .
	manualset3
147115	1	409590	5	NULL	NULL	0	NULL	discrimination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The discrimination was not acquired when sucrose presentations ( 9 or 18 ) also occurred during saline sessions .
	manualset3
147116	2	409590	5	NULL	NULL	0	NULL	sucrose presentations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The discrimination was not acquired when sucrose presentations ( 9 or 18 ) also occurred during saline sessions .
	manualset3
147117	3	409590	5	NULL	NULL	0	NULL	 9 or 18 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The discrimination was not acquired when sucrose presentations ( 9 or 18 ) also occurred during saline sessions .
	manualset3
147118	4	409590	5	NULL	NULL	0	NULL	saline sessions	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The discrimination was not acquired when sucrose presentations ( 9 or 18 ) also occurred during saline sessions .
	manualset3
147119	1	409591	5	NULL	NULL	0	NULL	discriminative stimulus effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The discriminative stimulus effects of cocaine were studied in rats trained to discriminate 10.0 mg/kg cocaine from vehicle in a shock avoidance paradigm .
	manualset3
147120	2	409591	5	NULL	NULL	0	NULL	cocaine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The discriminative stimulus effects of cocaine were studied in rats trained to discriminate 10.0 mg/kg cocaine from vehicle in a shock avoidance paradigm .
	manualset3
147121	3	409591	5	NULL	NULL	0	NULL	rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The discriminative stimulus effects of cocaine were studied in rats trained to discriminate 10.0 mg/kg cocaine from vehicle in a shock avoidance paradigm .
	manualset3
147122	4	409591	5	NULL	NULL	0	NULL	10.0 mg/kg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The discriminative stimulus effects of cocaine were studied in rats trained to discriminate 10.0 mg/kg cocaine from vehicle in a shock avoidance paradigm .
	manualset3
147123	5	409591	5	NULL	NULL	0	NULL	cocaine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The discriminative stimulus effects of cocaine were studied in rats trained to discriminate 10.0 mg/kg cocaine from vehicle in a shock avoidance paradigm .
	manualset3
147124	6	409591	5	NULL	NULL	0	NULL	vehicle 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The discriminative stimulus effects of cocaine were studied in rats trained to discriminate 10.0 mg/kg cocaine from vehicle in a shock avoidance paradigm .
	manualset3
147125	7	409591	5	NULL	NULL	0	NULL	shock avoidance paradigm	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The discriminative stimulus effects of cocaine were studied in rats trained to discriminate 10.0 mg/kg cocaine from vehicle in a shock avoidance paradigm .
	manualset3
147126	1	409592	5	NULL	NULL	0	NULL	disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The disease spreads rapidly between animals , and to ensure a window of opportunity for such spread , the virus has evolved multiple mechanisms to subvert the early immune response .
	manualset3
147127	2	409592	5	NULL	NULL	0	NULL	animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The disease spreads rapidly between animals , and to ensure a window of opportunity for such spread , the virus has evolved multiple mechanisms to subvert the early immune response .
	manualset3
147128	3	409592	5	NULL	NULL	0	NULL	window of opportunity	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The disease spreads rapidly between animals , and to ensure a window of opportunity for such spread , the virus has evolved multiple mechanisms to subvert the early immune response .
	manualset3
147129	4	409592	5	NULL	NULL	0	NULL	virus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The disease spreads rapidly between animals , and to ensure a window of opportunity for such spread , the virus has evolved multiple mechanisms to subvert the early immune response .
	manualset3
147130	5	409592	5	NULL	NULL	0	NULL	multiple mechanisms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The disease spreads rapidly between animals , and to ensure a window of opportunity for such spread , the virus has evolved multiple mechanisms to subvert the early immune response .
	manualset3
147131	6	409592	5	NULL	NULL	NULL	NULL	early immune response	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The disease spreads rapidly between animals , and to ensure a window of opportunity for such spread , the virus has evolved multiple mechanisms to subvert the early immune response .
	manualset3
147132	1	409593	5	NULL	NULL	0	NULL	dispersed sale	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dispersed sale of the cheese resulted in a regional dissemination of the organism and people were affected in eight townships .
	manualset3
147133	2	409593	5	NULL	NULL	0	NULL	cheese 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The dispersed sale of the cheese resulted in a regional dissemination of the organism and people were affected in eight townships .
	manualset3
147134	3	409593	5	NULL	NULL	0	NULL	regional dissemination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dispersed sale of the cheese resulted in a regional dissemination of the organism and people were affected in eight townships .
	manualset3
147135	4	409593	5	NULL	NULL	0	NULL	organism 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The dispersed sale of the cheese resulted in a regional dissemination of the organism and people were affected in eight townships .
	manualset3
147136	5	409593	5	NULL	NULL	0	NULL	people 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The dispersed sale of the cheese resulted in a regional dissemination of the organism and people were affected in eight townships .
	manualset3
147137	6	409593	5	NULL	NULL	0	NULL	eight townships 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The dispersed sale of the cheese resulted in a regional dissemination of the organism and people were affected in eight townships .
	manualset3
147138	1	409594	5	NULL	NULL	0	NULL	dissemination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissemination of information on the asymptomatic nature of HIV infection could potentially be very important in forming risk perception , awareness , and their willingness to participate in HIV interventions .
	manualset3
147139	2	409594	5	NULL	NULL	0	NULL	information 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissemination of information on the asymptomatic nature of HIV infection could potentially be very important in forming risk perception , awareness , and their willingness to participate in HIV interventions .
	manualset3
147140	3	409594	5	NULL	NULL	0	NULL	asymptomatic nature	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissemination of information on the asymptomatic nature of HIV infection could potentially be very important in forming risk perception , awareness , and their willingness to participate in HIV interventions .
	manualset3
147141	4	409594	5	NULL	NULL	0	NULL	HIV infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissemination of information on the asymptomatic nature of HIV infection could potentially be very important in forming risk perception , awareness , and their willingness to participate in HIV interventions .
	manualset3
147142	5	409594	5	NULL	NULL	NULL	NULL	risk perception	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The dissemination of information on the asymptomatic nature of HIV infection could potentially be very important in forming risk perception , awareness , and their willingness to participate in HIV interventions .
	manualset3
147143	6	409594	5	NULL	NULL	0	NULL	awareness 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissemination of information on the asymptomatic nature of HIV infection could potentially be very important in forming risk perception , awareness , and their willingness to participate in HIV interventions .
	manualset3
147144	7	409594	5	NULL	NULL	0	NULL	HIV interventions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissemination of information on the asymptomatic nature of HIV infection could potentially be very important in forming risk perception , awareness , and their willingness to participate in HIV interventions .
	manualset3
147145	1	409595	5	NULL	NULL	0	NULL	slender refrigeration probe	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A slender refrigeration probe for the production of reversible discrete lesions within the central nervous system of man and experimental animals is described .
	manualset3
147146	2	409595	5	NULL	NULL	0	NULL	production 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A slender refrigeration probe for the production of reversible discrete lesions within the central nervous system of man and experimental animals is described .
	manualset3
147147	3	409595	5	NULL	NULL	0	NULL	reversible discrete lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A slender refrigeration probe for the production of reversible discrete lesions within the central nervous system of man and experimental animals is described .
	manualset3
147148	4	409595	5	NULL	NULL	0	NULL	central nervous system 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A slender refrigeration probe for the production of reversible discrete lesions within the central nervous system of man and experimental animals is described .
	manualset3
147149	5	409595	5	NULL	NULL	0	NULL	man 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A slender refrigeration probe for the production of reversible discrete lesions within the central nervous system of man and experimental animals is described .
	manualset3
147150	6	409595	5	NULL	NULL	0	NULL	experimental animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A slender refrigeration probe for the production of reversible discrete lesions within the central nervous system of man and experimental animals is described .
	manualset3
147151	1	409596	5	NULL	NULL	0	NULL	dissipation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissipation of propamocarb-hydrochloride in tomatoes , potatoes and cucumber were evaluated .
	manualset3
147152	2	409596	5	NULL	NULL	0	NULL	propamocarb-hydrochloride	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissipation of propamocarb-hydrochloride in tomatoes , potatoes and cucumber were evaluated .
	manualset3
147153	3	409596	5	NULL	NULL	NULL	NULL	tomatoes 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The dissipation of propamocarb-hydrochloride in tomatoes , potatoes and cucumber were evaluated .
	manualset3
147154	4	409596	5	NULL	NULL	0	NULL	potatoes 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissipation of propamocarb-hydrochloride in tomatoes , potatoes and cucumber were evaluated .
	manualset3
147155	5	409596	5	NULL	NULL	0	NULL	cucumber 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissipation of propamocarb-hydrochloride in tomatoes , potatoes and cucumber were evaluated .
	manualset3
147156	1	409597	5	NULL	NULL	0	NULL	dissociation constant ( K ( D ) ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissociation constant ( K ( D ) ) was determined by surface plasmon resonance ( SPR ) analysis and was found to be 3.3910 ( -8 ) M and 8.610 ( -8 ) M for YWCS and baicalein ( positive control ) , respectively .
	manualset3
147157	2	409597	5	NULL	NULL	0	NULL	surface plasmon resonance ( SPR ) analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissociation constant ( K ( D ) ) was determined by surface plasmon resonance ( SPR ) analysis and was found to be 3.3910 ( -8 ) M and 8.610 ( -8 ) M for YWCS and baicalein ( positive control ) , respectively .
	manualset3
147158	3	409597	5	NULL	NULL	0	NULL	 3.3910 ( -8 ) M 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissociation constant ( K ( D ) ) was determined by surface plasmon resonance ( SPR ) analysis and was found to be 3.3910 ( -8 ) M and 8.610 ( -8 ) M for YWCS and baicalein ( positive control ) , respectively .
	manualset3
147159	4	409597	5	NULL	NULL	0	NULL	8.610 ( -8 ) M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissociation constant ( K ( D ) ) was determined by surface plasmon resonance ( SPR ) analysis and was found to be 3.3910 ( -8 ) M and 8.610 ( -8 ) M for YWCS and baicalein ( positive control ) , respectively .
	manualset3
147160	5	409597	5	NULL	NULL	NULL	NULL	YWCS 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The dissociation constant ( K ( D ) ) was determined by surface plasmon resonance ( SPR ) analysis and was found to be 3.3910 ( -8 ) M and 8.610 ( -8 ) M for YWCS and baicalein ( positive control ) , respectively .
	manualset3
147161	6	409597	5	NULL	NULL	0	NULL	baicalein ( positive control )	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissociation constant ( K ( D ) ) was determined by surface plasmon resonance ( SPR ) analysis and was found to be 3.3910 ( -8 ) M and 8.610 ( -8 ) M for YWCS and baicalein ( positive control ) , respectively .
	manualset3
147162	1	409598	5	NULL	NULL	0	NULL	dissociation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissociation induced by 5-HT ( 100 microM ) , paroxetine ( 0.15 microM ) , clomipramine ( 1 microM ) , citalopram ( 1 microM ) , imipramine ( 1 microM ) , or norzimeldine ( 1 microM ) was consistent with first-order dissociation kinetics with half-life values of dissociation ( t1/2 ) between 130 and 140 min .
	manualset3
147163	2	409598	5	NULL	NULL	0	NULL	5-HT	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissociation induced by 5-HT ( 100 microM ) , paroxetine ( 0.15 microM ) , clomipramine ( 1 microM ) , citalopram ( 1 microM ) , imipramine ( 1 microM ) , or norzimeldine ( 1 microM ) was consistent with first-order dissociation kinetics with half-life values of dissociation ( t1/2 ) between 130 and 140 min .
	manualset3
147164	3	409598	5	NULL	NULL	0	NULL	100 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissociation induced by 5-HT ( 100 microM ) , paroxetine ( 0.15 microM ) , clomipramine ( 1 microM ) , citalopram ( 1 microM ) , imipramine ( 1 microM ) , or norzimeldine ( 1 microM ) was consistent with first-order dissociation kinetics with half-life values of dissociation ( t1/2 ) between 130 and 140 min .
	manualset3
147165	4	409598	5	NULL	NULL	0	NULL	paroxetine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissociation induced by 5-HT ( 100 microM ) , paroxetine ( 0.15 microM ) , clomipramine ( 1 microM ) , citalopram ( 1 microM ) , imipramine ( 1 microM ) , or norzimeldine ( 1 microM ) was consistent with first-order dissociation kinetics with half-life values of dissociation ( t1/2 ) between 130 and 140 min .
	manualset3
147166	5	409598	5	NULL	NULL	0	NULL	 0.15 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissociation induced by 5-HT ( 100 microM ) , paroxetine ( 0.15 microM ) , clomipramine ( 1 microM ) , citalopram ( 1 microM ) , imipramine ( 1 microM ) , or norzimeldine ( 1 microM ) was consistent with first-order dissociation kinetics with half-life values of dissociation ( t1/2 ) between 130 and 140 min .
	manualset3
147167	6	409598	5	NULL	NULL	0	NULL	clomipramine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissociation induced by 5-HT ( 100 microM ) , paroxetine ( 0.15 microM ) , clomipramine ( 1 microM ) , citalopram ( 1 microM ) , imipramine ( 1 microM ) , or norzimeldine ( 1 microM ) was consistent with first-order dissociation kinetics with half-life values of dissociation ( t1/2 ) between 130 and 140 min .
	manualset3
147168	7	409598	5	NULL	NULL	0	NULL	1 microM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissociation induced by 5-HT ( 100 microM ) , paroxetine ( 0.15 microM ) , clomipramine ( 1 microM ) , citalopram ( 1 microM ) , imipramine ( 1 microM ) , or norzimeldine ( 1 microM ) was consistent with first-order dissociation kinetics with half-life values of dissociation ( t1/2 ) between 130 and 140 min .
	manualset3
147169	8	409598	5	NULL	NULL	0	NULL	citalopram 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissociation induced by 5-HT ( 100 microM ) , paroxetine ( 0.15 microM ) , clomipramine ( 1 microM ) , citalopram ( 1 microM ) , imipramine ( 1 microM ) , or norzimeldine ( 1 microM ) was consistent with first-order dissociation kinetics with half-life values of dissociation ( t1/2 ) between 130 and 140 min .
	manualset3
147170	9	409598	5	NULL	NULL	0	NULL	1 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissociation induced by 5-HT ( 100 microM ) , paroxetine ( 0.15 microM ) , clomipramine ( 1 microM ) , citalopram ( 1 microM ) , imipramine ( 1 microM ) , or norzimeldine ( 1 microM ) was consistent with first-order dissociation kinetics with half-life values of dissociation ( t1/2 ) between 130 and 140 min .
	manualset3
147171	10	409598	5	NULL	NULL	0	NULL	imipramine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissociation induced by 5-HT ( 100 microM ) , paroxetine ( 0.15 microM ) , clomipramine ( 1 microM ) , citalopram ( 1 microM ) , imipramine ( 1 microM ) , or norzimeldine ( 1 microM ) was consistent with first-order dissociation kinetics with half-life values of dissociation ( t1/2 ) between 130 and 140 min .
	manualset3
147172	11	409598	5	NULL	NULL	0	NULL	1 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissociation induced by 5-HT ( 100 microM ) , paroxetine ( 0.15 microM ) , clomipramine ( 1 microM ) , citalopram ( 1 microM ) , imipramine ( 1 microM ) , or norzimeldine ( 1 microM ) was consistent with first-order dissociation kinetics with half-life values of dissociation ( t1/2 ) between 130 and 140 min .
	manualset3
147173	12	409598	5	NULL	NULL	0	NULL	norzimeldine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissociation induced by 5-HT ( 100 microM ) , paroxetine ( 0.15 microM ) , clomipramine ( 1 microM ) , citalopram ( 1 microM ) , imipramine ( 1 microM ) , or norzimeldine ( 1 microM ) was consistent with first-order dissociation kinetics with half-life values of dissociation ( t1/2 ) between 130 and 140 min .
	manualset3
147174	13	409598	5	NULL	NULL	0	NULL	 1 microM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissociation induced by 5-HT ( 100 microM ) , paroxetine ( 0.15 microM ) , clomipramine ( 1 microM ) , citalopram ( 1 microM ) , imipramine ( 1 microM ) , or norzimeldine ( 1 microM ) was consistent with first-order dissociation kinetics with half-life values of dissociation ( t1/2 ) between 130 and 140 min .
	manualset3
147175	14	409598	5	NULL	NULL	0	NULL	 first-order dissociation kinetics 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissociation induced by 5-HT ( 100 microM ) , paroxetine ( 0.15 microM ) , clomipramine ( 1 microM ) , citalopram ( 1 microM ) , imipramine ( 1 microM ) , or norzimeldine ( 1 microM ) was consistent with first-order dissociation kinetics with half-life values of dissociation ( t1/2 ) between 130 and 140 min .
	manualset3
147176	15	409598	5	NULL	NULL	0	NULL	half-life values of dissociation ( t1/2 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissociation induced by 5-HT ( 100 microM ) , paroxetine ( 0.15 microM ) , clomipramine ( 1 microM ) , citalopram ( 1 microM ) , imipramine ( 1 microM ) , or norzimeldine ( 1 microM ) was consistent with first-order dissociation kinetics with half-life values of dissociation ( t1/2 ) between 130 and 140 min .
	manualset3
147177	16	409598	5	NULL	NULL	0	NULL	130 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissociation induced by 5-HT ( 100 microM ) , paroxetine ( 0.15 microM ) , clomipramine ( 1 microM ) , citalopram ( 1 microM ) , imipramine ( 1 microM ) , or norzimeldine ( 1 microM ) was consistent with first-order dissociation kinetics with half-life values of dissociation ( t1/2 ) between 130 and 140 min .
	manualset3
147178	17	409598	5	NULL	NULL	0	NULL	 140 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The dissociation induced by 5-HT ( 100 microM ) , paroxetine ( 0.15 microM ) , clomipramine ( 1 microM ) , citalopram ( 1 microM ) , imipramine ( 1 microM ) , or norzimeldine ( 1 microM ) was consistent with first-order dissociation kinetics with half-life values of dissociation ( t1/2 ) between 130 and 140 min .
	manualset3
147179	1	409599	5	NULL	NULL	0	NULL	distance 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The distance between neighboring peaks in the SRP for individual RAs and SAs was approximately the same as the distance between the peaks of the wavy surface .
	manualset3
147180	2	409599	5	NULL	NULL	0	NULL	neighboring peaks 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The distance between neighboring peaks in the SRP for individual RAs and SAs was approximately the same as the distance between the peaks of the wavy surface .
	manualset3
147181	3	409599	5	NULL	NULL	0	NULL	SRP 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The distance between neighboring peaks in the SRP for individual RAs and SAs was approximately the same as the distance between the peaks of the wavy surface .
	manualset3
147182	4	409599	5	NULL	NULL	0	NULL	RAs 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The distance between neighboring peaks in the SRP for individual RAs and SAs was approximately the same as the distance between the peaks of the wavy surface .
	manualset3
147183	5	409599	5	NULL	NULL	0	NULL	SAs 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The distance between neighboring peaks in the SRP for individual RAs and SAs was approximately the same as the distance between the peaks of the wavy surface .
	manualset3
147184	6	409599	5	NULL	NULL	0	NULL	distance 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The distance between neighboring peaks in the SRP for individual RAs and SAs was approximately the same as the distance between the peaks of the wavy surface .
	manualset3
147185	7	409599	5	NULL	NULL	0	NULL	peaks 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The distance between neighboring peaks in the SRP for individual RAs and SAs was approximately the same as the distance between the peaks of the wavy surface .
	manualset3
147186	8	409599	5	NULL	NULL	0	NULL	wavy surface	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The distance between neighboring peaks in the SRP for individual RAs and SAs was approximately the same as the distance between the peaks of the wavy surface .
	manualset3
147187	1	409600	5	NULL	NULL	0	NULL	distance 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The distance traveled by vanguard sperm was affected by an interaction of the photoperiod and temperature ( P & lt ; 0.001 ) .
	manualset3
147188	2	409600	5	NULL	NULL	0	NULL	vanguard sperm	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The distance traveled by vanguard sperm was affected by an interaction of the photoperiod and temperature ( P & lt ; 0.001 ) .
	manualset3
147189	3	409600	5	NULL	NULL	0	NULL	interaction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The distance traveled by vanguard sperm was affected by an interaction of the photoperiod and temperature ( P & lt ; 0.001 ) .
	manualset3
147190	4	409600	5	NULL	NULL	0	NULL	photoperiod 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The distance traveled by vanguard sperm was affected by an interaction of the photoperiod and temperature ( P & lt ; 0.001 ) .
	manualset3
147191	5	409600	5	NULL	NULL	0	NULL	temperature 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The distance traveled by vanguard sperm was affected by an interaction of the photoperiod and temperature ( P & lt ; 0.001 ) .
	manualset3
147192	6	409600	5	NULL	NULL	0	NULL	 P & lt ; 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The distance traveled by vanguard sperm was affected by an interaction of the photoperiod and temperature ( P & lt ; 0.001 ) .
	manualset3
147193	1	409601	5	NULL	NULL	0	NULL	distinction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The distinction between Tc1 and gambol is also consistent with the unique TIRs in gambol elements and the presence of a ` W ( I/L/V ) DEDC ' signature near their N-termini .
	manualset3
147194	2	409601	5	NULL	NULL	0	NULL	Tc1 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The distinction between Tc1 and gambol is also consistent with the unique TIRs in gambol elements and the presence of a ` W ( I/L/V ) DEDC ' signature near their N-termini .
	manualset3
147195	3	409601	5	NULL	NULL	0	NULL	gambol 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The distinction between Tc1 and gambol is also consistent with the unique TIRs in gambol elements and the presence of a ` W ( I/L/V ) DEDC ' signature near their N-termini .
	manualset3
147196	4	409601	5	NULL	NULL	0	NULL	TIRs 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The distinction between Tc1 and gambol is also consistent with the unique TIRs in gambol elements and the presence of a ` W ( I/L/V ) DEDC ' signature near their N-termini .
	manualset3
147197	5	409601	5	NULL	NULL	0	NULL	gambol elements 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The distinction between Tc1 and gambol is also consistent with the unique TIRs in gambol elements and the presence of a ` W ( I/L/V ) DEDC ' signature near their N-termini .
	manualset3
147198	6	409601	5	NULL	NULL	0	NULL	` W ( I/L/V ) DEDC ' signature	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The distinction between Tc1 and gambol is also consistent with the unique TIRs in gambol elements and the presence of a ` W ( I/L/V ) DEDC ' signature near their N-termini .
	manualset3
147199	7	409601	5	NULL	NULL	0	NULL	 N-termini 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The distinction between Tc1 and gambol is also consistent with the unique TIRs in gambol elements and the presence of a ` W ( I/L/V ) DEDC ' signature near their N-termini .
	manualset3
147201	2	409602	5	NULL	NULL	0	NULL	distorted cognitions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The distorted cognitions are supported by maladaptive cognitive schemata , which involve immature `` either-or '' rules of conduct or inflexible and unattainable self-expectations .
	manualset3
147202	3	409602	5	NULL	NULL	0	NULL	maladaptive cognitive schemata	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The distorted cognitions are supported by maladaptive cognitive schemata , which involve immature `` either-or '' rules of conduct or inflexible and unattainable self-expectations .
	manualset3
147203	4	409602	5	NULL	NULL	0	NULL	immature `` either-or '' rules of conduct	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The distorted cognitions are supported by maladaptive cognitive schemata , which involve immature `` either-or '' rules of conduct or inflexible and unattainable self-expectations .
	manualset3
147204	5	409602	5	NULL	NULL	0	NULL	inflexible and unattainable self-expectations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The distorted cognitions are supported by maladaptive cognitive schemata , which involve immature `` either-or '' rules of conduct or inflexible and unattainable self-expectations .
	manualset3
147205	1	409603	5	NULL	NULL	0	NULL	systemic blood pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A slight increase followed by a decrease was observed in systemic blood pressure and LV systolic pressure .
	manualset3
147206	2	409603	5	NULL	NULL	0	NULL	LV systolic pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A slight increase followed by a decrease was observed in systemic blood pressure and LV systolic pressure .
	manualset3
147207	1	409604	5	NULL	NULL	0	NULL	distribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution and function of phosphatidylserine in cellular membranes .
	manualset3
147208	2	409604	5	NULL	NULL	0	NULL	function 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution and function of phosphatidylserine in cellular membranes .
	manualset3
147209	3	409604	5	NULL	NULL	0	NULL	phosphatidylserine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution and function of phosphatidylserine in cellular membranes .
	manualset3
147210	4	409604	5	NULL	NULL	0	NULL	cellular membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution and function of phosphatidylserine in cellular membranes .
	manualset3
147211	1	409605	5	NULL	NULL	0	NULL	distribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution and numbers of leucocytes and mast cells ( MC ) in the canine gastrointestinal tract of three different age groups was investigated immunhistochemically .
	manualset3
147212	2	409605	5	NULL	NULL	0	NULL	numbers 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution and numbers of leucocytes and mast cells ( MC ) in the canine gastrointestinal tract of three different age groups was investigated immunhistochemically .
	manualset3
147213	3	409605	5	NULL	NULL	0	NULL	leucocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution and numbers of leucocytes and mast cells ( MC ) in the canine gastrointestinal tract of three different age groups was investigated immunhistochemically .
	manualset3
147214	4	409605	5	NULL	NULL	0	NULL	mast cells ( MC ) 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution and numbers of leucocytes and mast cells ( MC ) in the canine gastrointestinal tract of three different age groups was investigated immunhistochemically .
	manualset3
147215	5	409605	5	NULL	NULL	0	NULL	canine gastrointestinal tract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution and numbers of leucocytes and mast cells ( MC ) in the canine gastrointestinal tract of three different age groups was investigated immunhistochemically .
	manualset3
147216	6	409605	5	NULL	NULL	0	NULL	three 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution and numbers of leucocytes and mast cells ( MC ) in the canine gastrointestinal tract of three different age groups was investigated immunhistochemically .
	manualset3
147217	7	409605	5	NULL	NULL	0	NULL	age groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution and numbers of leucocytes and mast cells ( MC ) in the canine gastrointestinal tract of three different age groups was investigated immunhistochemically .
	manualset3
147218	1	409606	5	NULL	NULL	0	NULL	distribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of CTLA-4 exon 1 A ( 49 ) G genotype , phenotype and allele frequencies did not differ between patients with MS and healthy subjects .
	manualset3
147219	2	409606	5	NULL	NULL	0	NULL	CTLA-4 exon 1 A ( 49 ) G genotype	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of CTLA-4 exon 1 A ( 49 ) G genotype , phenotype and allele frequencies did not differ between patients with MS and healthy subjects .
	manualset3
147220	3	409606	5	NULL	NULL	0	NULL	phenotype 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of CTLA-4 exon 1 A ( 49 ) G genotype , phenotype and allele frequencies did not differ between patients with MS and healthy subjects .
	manualset3
147221	4	409606	5	NULL	NULL	0	NULL	allele frequencies	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of CTLA-4 exon 1 A ( 49 ) G genotype , phenotype and allele frequencies did not differ between patients with MS and healthy subjects .
	manualset3
147222	5	409606	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of CTLA-4 exon 1 A ( 49 ) G genotype , phenotype and allele frequencies did not differ between patients with MS and healthy subjects .
	manualset3
147223	6	409606	5	NULL	NULL	0	NULL	MS subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of CTLA-4 exon 1 A ( 49 ) G genotype , phenotype and allele frequencies did not differ between patients with MS and healthy subjects .
	manualset3
147224	7	409606	5	NULL	NULL	0	NULL	healthy subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of CTLA-4 exon 1 A ( 49 ) G genotype , phenotype and allele frequencies did not differ between patients with MS and healthy subjects .
	manualset3
147225	1	409607	5	NULL	NULL	0	NULL	distribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of DNA and RNA change gradually in nuclei as epidermal cells differentiate .
	manualset3
147226	2	409607	5	NULL	NULL	0	NULL	DNA change	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of DNA and RNA change gradually in nuclei as epidermal cells differentiate .
	manualset3
147227	3	409607	5	NULL	NULL	0	NULL	RNA change	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of DNA and RNA change gradually in nuclei as epidermal cells differentiate .
	manualset3
147228	4	409607	5	NULL	NULL	0	NULL	nuclei 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of DNA and RNA change gradually in nuclei as epidermal cells differentiate .
	manualset3
147229	5	409607	5	NULL	NULL	0	NULL	epidermal cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of DNA and RNA change gradually in nuclei as epidermal cells differentiate .
	manualset3
147230	1	409608	5	NULL	NULL	0	NULL	distribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of actin and cytokeratin filaments , as well as 51chromium ( 51Cr ) release and trypan blue dye exclusion were assessed .
	manualset3
147231	2	409608	5	NULL	NULL	0	NULL	actin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of actin and cytokeratin filaments , as well as 51chromium ( 51Cr ) release and trypan blue dye exclusion were assessed .
	manualset3
147232	3	409608	5	NULL	NULL	0	NULL	cytokeratin filaments 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of actin and cytokeratin filaments , as well as 51chromium ( 51Cr ) release and trypan blue dye exclusion were assessed .
	manualset3
147233	4	409608	5	NULL	NULL	0	NULL	51chromium ( 51Cr ) release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of actin and cytokeratin filaments , as well as 51chromium ( 51Cr ) release and trypan blue dye exclusion were assessed .
	manualset3
147234	5	409608	5	NULL	NULL	0	NULL	trypan blue dye exclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of actin and cytokeratin filaments , as well as 51chromium ( 51Cr ) release and trypan blue dye exclusion were assessed .
	manualset3
147235	1	409609	5	NULL	NULL	0	NULL	distribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of patients between pain groups was as follows ; nine had nociceptive pain , two suffered neuropathic pain , there were no placebo responders and seven were non-responders .
	manualset3
147236	2	409609	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of patients between pain groups was as follows ; nine had nociceptive pain , two suffered neuropathic pain , there were no placebo responders and seven were non-responders .
	manualset3
147237	3	409609	5	NULL	NULL	0	NULL	pain groups 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of patients between pain groups was as follows ; nine had nociceptive pain , two suffered neuropathic pain , there were no placebo responders and seven were non-responders .
	manualset3
147238	4	409609	5	NULL	NULL	0	NULL	nine 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of patients between pain groups was as follows ; nine had nociceptive pain , two suffered neuropathic pain , there were no placebo responders and seven were non-responders .
	manualset3
147239	5	409609	5	NULL	NULL	0	NULL	nociceptive pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of patients between pain groups was as follows ; nine had nociceptive pain , two suffered neuropathic pain , there were no placebo responders and seven were non-responders .
	manualset3
147240	6	409609	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of patients between pain groups was as follows ; nine had nociceptive pain , two suffered neuropathic pain , there were no placebo responders and seven were non-responders .
	manualset3
147241	7	409609	5	NULL	NULL	0	NULL	neuropathic pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of patients between pain groups was as follows ; nine had nociceptive pain , two suffered neuropathic pain , there were no placebo responders and seven were non-responders .
	manualset3
147242	8	409609	5	NULL	NULL	0	NULL	placebo responders	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of patients between pain groups was as follows ; nine had nociceptive pain , two suffered neuropathic pain , there were no placebo responders and seven were non-responders .
	manualset3
147243	9	409609	5	NULL	NULL	0	NULL	seven 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of patients between pain groups was as follows ; nine had nociceptive pain , two suffered neuropathic pain , there were no placebo responders and seven were non-responders .
	manualset3
147244	10	409609	5	NULL	NULL	0	NULL	non-responders	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of patients between pain groups was as follows ; nine had nociceptive pain , two suffered neuropathic pain , there were no placebo responders and seven were non-responders .
	manualset3
147245	1	409610	5	NULL	NULL	0	NULL	distribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of polymorphic restriction fragments among the CXB set of recombinant inbred ( RI ) strains demonstrates the feasibility of using these probes for chromosome mapping .
	manualset3
147246	2	409610	5	NULL	NULL	0	NULL	polymorphic restriction fragments	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of polymorphic restriction fragments among the CXB set of recombinant inbred ( RI ) strains demonstrates the feasibility of using these probes for chromosome mapping .
	manualset3
147247	3	409610	5	NULL	NULL	0	NULL	CXB set	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of polymorphic restriction fragments among the CXB set of recombinant inbred ( RI ) strains demonstrates the feasibility of using these probes for chromosome mapping .
	manualset3
147248	4	409610	5	NULL	NULL	0	NULL	recombinant inbred ( RI ) strains 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of polymorphic restriction fragments among the CXB set of recombinant inbred ( RI ) strains demonstrates the feasibility of using these probes for chromosome mapping .
	manualset3
147249	5	409610	5	NULL	NULL	0	NULL	feasibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of polymorphic restriction fragments among the CXB set of recombinant inbred ( RI ) strains demonstrates the feasibility of using these probes for chromosome mapping .
	manualset3
147250	6	409610	5	NULL	NULL	0	NULL	probes 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of polymorphic restriction fragments among the CXB set of recombinant inbred ( RI ) strains demonstrates the feasibility of using these probes for chromosome mapping .
	manualset3
147251	7	409610	5	NULL	NULL	0	NULL	chromosome mapping	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of polymorphic restriction fragments among the CXB set of recombinant inbred ( RI ) strains demonstrates the feasibility of using these probes for chromosome mapping .
	manualset3
147252	1	409611	5	NULL	NULL	0	NULL	distribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of portable technology that has been traditionally managed by the materials management function is a logical match to the expanding role of clinical engineering departments in technology management .
	manualset3
147253	2	409611	5	NULL	NULL	0	NULL	portable technology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of portable technology that has been traditionally managed by the materials management function is a logical match to the expanding role of clinical engineering departments in technology management .
	manualset3
147254	3	409611	5	NULL	NULL	0	NULL	materials management function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of portable technology that has been traditionally managed by the materials management function is a logical match to the expanding role of clinical engineering departments in technology management .
	manualset3
147255	4	409611	5	NULL	NULL	0	NULL	logical match	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of portable technology that has been traditionally managed by the materials management function is a logical match to the expanding role of clinical engineering departments in technology management .
	manualset3
147256	5	409611	5	NULL	NULL	0	NULL	expanding role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of portable technology that has been traditionally managed by the materials management function is a logical match to the expanding role of clinical engineering departments in technology management .
	manualset3
147257	6	409611	5	NULL	NULL	0	NULL	clinical engineering departments	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of portable technology that has been traditionally managed by the materials management function is a logical match to the expanding role of clinical engineering departments in technology management .
	manualset3
147258	7	409611	5	NULL	NULL	0	NULL	technology management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of portable technology that has been traditionally managed by the materials management function is a logical match to the expanding role of clinical engineering departments in technology management .
	manualset3
147259	1	409612	5	NULL	NULL	0	NULL	slight negative effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A slight negative effect on HaCaT cells was noted in vitro which is most likely due to the Ca ( 2 + ) deprivation of the medium by binding to the SAP .
	manualset3
147260	2	409612	5	NULL	NULL	0	NULL	HaCaT cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A slight negative effect on HaCaT cells was noted in vitro which is most likely due to the Ca ( 2 + ) deprivation of the medium by binding to the SAP .
	manualset3
147261	3	409612	5	NULL	NULL	0	NULL	 Ca ( 2 + ) deprivation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A slight negative effect on HaCaT cells was noted in vitro which is most likely due to the Ca ( 2 + ) deprivation of the medium by binding to the SAP .
	manualset3
147262	4	409612	5	NULL	NULL	0	NULL	medium 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A slight negative effect on HaCaT cells was noted in vitro which is most likely due to the Ca ( 2 + ) deprivation of the medium by binding to the SAP .
	manualset3
147263	5	409612	5	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A slight negative effect on HaCaT cells was noted in vitro which is most likely due to the Ca ( 2 + ) deprivation of the medium by binding to the SAP .
	manualset3
147264	6	409612	5	NULL	NULL	0	NULL	SAP 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A slight negative effect on HaCaT cells was noted in vitro which is most likely due to the Ca ( 2 + ) deprivation of the medium by binding to the SAP .
	manualset3
147265	1	409613	5	NULL	NULL	0	NULL	distribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of total nuclear receptors within each nuclear compartment was ( percentage of nucleoplasmic , hypertonic salt-extractable , and salt-resistant receptors ) : Cerebrum : 23.6 , 52.2 , 24.2 ; Liver : 25.2 , 57.2 , 17.5 ; Kidney : 45.9 , 33.5 , 20.6 ; Testis : 65.5 , 14.7 , 19.7 ; and Spleen : 66.7 , 18.7 , 14.6 .
	manualset3
147266	2	409613	5	NULL	NULL	0	NULL	total nuclear receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of total nuclear receptors within each nuclear compartment was ( percentage of nucleoplasmic , hypertonic salt-extractable , and salt-resistant receptors ) : Cerebrum : 23.6 , 52.2 , 24.2 ; Liver : 25.2 , 57.2 , 17.5 ; Kidney : 45.9 , 33.5 , 20.6 ; Testis : 65.5 , 14.7 , 19.7 ; and Spleen : 66.7 , 18.7 , 14.6 .
	manualset3
147267	3	409613	5	NULL	NULL	0	NULL	nuclear compartment 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of total nuclear receptors within each nuclear compartment was ( percentage of nucleoplasmic , hypertonic salt-extractable , and salt-resistant receptors ) : Cerebrum : 23.6 , 52.2 , 24.2 ; Liver : 25.2 , 57.2 , 17.5 ; Kidney : 45.9 , 33.5 , 20.6 ; Testis : 65.5 , 14.7 , 19.7 ; and Spleen : 66.7 , 18.7 , 14.6 .
	manualset3
147268	4	409613	5	NULL	NULL	0	NULL	percentage 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of total nuclear receptors within each nuclear compartment was ( percentage of nucleoplasmic , hypertonic salt-extractable , and salt-resistant receptors ) : Cerebrum : 23.6 , 52.2 , 24.2 ; Liver : 25.2 , 57.2 , 17.5 ; Kidney : 45.9 , 33.5 , 20.6 ; Testis : 65.5 , 14.7 , 19.7 ; and Spleen : 66.7 , 18.7 , 14.6 .
	manualset3
147269	5	409613	5	NULL	NULL	NULL	NULL	nucleoplasmic receptors	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The distribution of total nuclear receptors within each nuclear compartment was ( percentage of nucleoplasmic , hypertonic salt-extractable , and salt-resistant receptors ) : Cerebrum : 23.6 , 52.2 , 24.2 ; Liver : 25.2 , 57.2 , 17.5 ; Kidney : 45.9 , 33.5 , 20.6 ; Testis : 65.5 , 14.7 , 19.7 ; and Spleen : 66.7 , 18.7 , 14.6 .
	manualset3
147270	6	409613	5	NULL	NULL	0	NULL	hypertonic salt-extractable receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of total nuclear receptors within each nuclear compartment was ( percentage of nucleoplasmic , hypertonic salt-extractable , and salt-resistant receptors ) : Cerebrum : 23.6 , 52.2 , 24.2 ; Liver : 25.2 , 57.2 , 17.5 ; Kidney : 45.9 , 33.5 , 20.6 ; Testis : 65.5 , 14.7 , 19.7 ; and Spleen : 66.7 , 18.7 , 14.6 .
	manualset3
147271	7	409613	5	NULL	NULL	0	NULL	salt-resistant receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of total nuclear receptors within each nuclear compartment was ( percentage of nucleoplasmic , hypertonic salt-extractable , and salt-resistant receptors ) : Cerebrum : 23.6 , 52.2 , 24.2 ; Liver : 25.2 , 57.2 , 17.5 ; Kidney : 45.9 , 33.5 , 20.6 ; Testis : 65.5 , 14.7 , 19.7 ; and Spleen : 66.7 , 18.7 , 14.6 .
	manualset3
147272	8	409613	5	NULL	NULL	0	NULL	Cerebrum 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of total nuclear receptors within each nuclear compartment was ( percentage of nucleoplasmic , hypertonic salt-extractable , and salt-resistant receptors ) : Cerebrum : 23.6 , 52.2 , 24.2 ; Liver : 25.2 , 57.2 , 17.5 ; Kidney : 45.9 , 33.5 , 20.6 ; Testis : 65.5 , 14.7 , 19.7 ; and Spleen : 66.7 , 18.7 , 14.6 .
	manualset3
147273	9	409613	5	NULL	NULL	0	NULL	23.6	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of total nuclear receptors within each nuclear compartment was ( percentage of nucleoplasmic , hypertonic salt-extractable , and salt-resistant receptors ) : Cerebrum : 23.6 , 52.2 , 24.2 ; Liver : 25.2 , 57.2 , 17.5 ; Kidney : 45.9 , 33.5 , 20.6 ; Testis : 65.5 , 14.7 , 19.7 ; and Spleen : 66.7 , 18.7 , 14.6 .
	manualset3
147274	10	409613	5	NULL	NULL	0	NULL	52.2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of total nuclear receptors within each nuclear compartment was ( percentage of nucleoplasmic , hypertonic salt-extractable , and salt-resistant receptors ) : Cerebrum : 23.6 , 52.2 , 24.2 ; Liver : 25.2 , 57.2 , 17.5 ; Kidney : 45.9 , 33.5 , 20.6 ; Testis : 65.5 , 14.7 , 19.7 ; and Spleen : 66.7 , 18.7 , 14.6 .
	manualset3
147275	11	409613	5	NULL	NULL	0	NULL	24.2 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of total nuclear receptors within each nuclear compartment was ( percentage of nucleoplasmic , hypertonic salt-extractable , and salt-resistant receptors ) : Cerebrum : 23.6 , 52.2 , 24.2 ; Liver : 25.2 , 57.2 , 17.5 ; Kidney : 45.9 , 33.5 , 20.6 ; Testis : 65.5 , 14.7 , 19.7 ; and Spleen : 66.7 , 18.7 , 14.6 .
	manualset3
147276	12	409613	5	NULL	NULL	0	NULL	Liver 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of total nuclear receptors within each nuclear compartment was ( percentage of nucleoplasmic , hypertonic salt-extractable , and salt-resistant receptors ) : Cerebrum : 23.6 , 52.2 , 24.2 ; Liver : 25.2 , 57.2 , 17.5 ; Kidney : 45.9 , 33.5 , 20.6 ; Testis : 65.5 , 14.7 , 19.7 ; and Spleen : 66.7 , 18.7 , 14.6 .
	manualset3
147277	13	409613	5	NULL	NULL	0	NULL	25.2 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of total nuclear receptors within each nuclear compartment was ( percentage of nucleoplasmic , hypertonic salt-extractable , and salt-resistant receptors ) : Cerebrum : 23.6 , 52.2 , 24.2 ; Liver : 25.2 , 57.2 , 17.5 ; Kidney : 45.9 , 33.5 , 20.6 ; Testis : 65.5 , 14.7 , 19.7 ; and Spleen : 66.7 , 18.7 , 14.6 .
	manualset3
147278	14	409613	5	NULL	NULL	0	NULL	 57.2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of total nuclear receptors within each nuclear compartment was ( percentage of nucleoplasmic , hypertonic salt-extractable , and salt-resistant receptors ) : Cerebrum : 23.6 , 52.2 , 24.2 ; Liver : 25.2 , 57.2 , 17.5 ; Kidney : 45.9 , 33.5 , 20.6 ; Testis : 65.5 , 14.7 , 19.7 ; and Spleen : 66.7 , 18.7 , 14.6 .
	manualset3
147279	15	409613	5	NULL	NULL	0	NULL	17.5	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of total nuclear receptors within each nuclear compartment was ( percentage of nucleoplasmic , hypertonic salt-extractable , and salt-resistant receptors ) : Cerebrum : 23.6 , 52.2 , 24.2 ; Liver : 25.2 , 57.2 , 17.5 ; Kidney : 45.9 , 33.5 , 20.6 ; Testis : 65.5 , 14.7 , 19.7 ; and Spleen : 66.7 , 18.7 , 14.6 .
	manualset3
147280	16	409613	5	NULL	NULL	0	NULL	Kidney 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of total nuclear receptors within each nuclear compartment was ( percentage of nucleoplasmic , hypertonic salt-extractable , and salt-resistant receptors ) : Cerebrum : 23.6 , 52.2 , 24.2 ; Liver : 25.2 , 57.2 , 17.5 ; Kidney : 45.9 , 33.5 , 20.6 ; Testis : 65.5 , 14.7 , 19.7 ; and Spleen : 66.7 , 18.7 , 14.6 .
	manualset3
147281	17	409613	5	NULL	NULL	0	NULL	45.9	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of total nuclear receptors within each nuclear compartment was ( percentage of nucleoplasmic , hypertonic salt-extractable , and salt-resistant receptors ) : Cerebrum : 23.6 , 52.2 , 24.2 ; Liver : 25.2 , 57.2 , 17.5 ; Kidney : 45.9 , 33.5 , 20.6 ; Testis : 65.5 , 14.7 , 19.7 ; and Spleen : 66.7 , 18.7 , 14.6 .
	manualset3
147282	18	409613	5	NULL	NULL	0	NULL	33.5	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of total nuclear receptors within each nuclear compartment was ( percentage of nucleoplasmic , hypertonic salt-extractable , and salt-resistant receptors ) : Cerebrum : 23.6 , 52.2 , 24.2 ; Liver : 25.2 , 57.2 , 17.5 ; Kidney : 45.9 , 33.5 , 20.6 ; Testis : 65.5 , 14.7 , 19.7 ; and Spleen : 66.7 , 18.7 , 14.6 .
	manualset3
147283	19	409613	5	NULL	NULL	0	NULL	20.6	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of total nuclear receptors within each nuclear compartment was ( percentage of nucleoplasmic , hypertonic salt-extractable , and salt-resistant receptors ) : Cerebrum : 23.6 , 52.2 , 24.2 ; Liver : 25.2 , 57.2 , 17.5 ; Kidney : 45.9 , 33.5 , 20.6 ; Testis : 65.5 , 14.7 , 19.7 ; and Spleen : 66.7 , 18.7 , 14.6 .
	manualset3
147284	20	409613	5	NULL	NULL	0	NULL	Testis 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of total nuclear receptors within each nuclear compartment was ( percentage of nucleoplasmic , hypertonic salt-extractable , and salt-resistant receptors ) : Cerebrum : 23.6 , 52.2 , 24.2 ; Liver : 25.2 , 57.2 , 17.5 ; Kidney : 45.9 , 33.5 , 20.6 ; Testis : 65.5 , 14.7 , 19.7 ; and Spleen : 66.7 , 18.7 , 14.6 .
	manualset3
147285	21	409613	5	NULL	NULL	0	NULL	65.5	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of total nuclear receptors within each nuclear compartment was ( percentage of nucleoplasmic , hypertonic salt-extractable , and salt-resistant receptors ) : Cerebrum : 23.6 , 52.2 , 24.2 ; Liver : 25.2 , 57.2 , 17.5 ; Kidney : 45.9 , 33.5 , 20.6 ; Testis : 65.5 , 14.7 , 19.7 ; and Spleen : 66.7 , 18.7 , 14.6 .
	manualset3
147286	22	409613	5	NULL	NULL	0	NULL	14.7	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of total nuclear receptors within each nuclear compartment was ( percentage of nucleoplasmic , hypertonic salt-extractable , and salt-resistant receptors ) : Cerebrum : 23.6 , 52.2 , 24.2 ; Liver : 25.2 , 57.2 , 17.5 ; Kidney : 45.9 , 33.5 , 20.6 ; Testis : 65.5 , 14.7 , 19.7 ; and Spleen : 66.7 , 18.7 , 14.6 .
	manualset3
147287	23	409613	5	NULL	NULL	0	NULL	19.7 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of total nuclear receptors within each nuclear compartment was ( percentage of nucleoplasmic , hypertonic salt-extractable , and salt-resistant receptors ) : Cerebrum : 23.6 , 52.2 , 24.2 ; Liver : 25.2 , 57.2 , 17.5 ; Kidney : 45.9 , 33.5 , 20.6 ; Testis : 65.5 , 14.7 , 19.7 ; and Spleen : 66.7 , 18.7 , 14.6 .
	manualset3
147288	24	409613	5	NULL	NULL	0	NULL	Spleen 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of total nuclear receptors within each nuclear compartment was ( percentage of nucleoplasmic , hypertonic salt-extractable , and salt-resistant receptors ) : Cerebrum : 23.6 , 52.2 , 24.2 ; Liver : 25.2 , 57.2 , 17.5 ; Kidney : 45.9 , 33.5 , 20.6 ; Testis : 65.5 , 14.7 , 19.7 ; and Spleen : 66.7 , 18.7 , 14.6 .
	manualset3
147289	25	409613	5	NULL	NULL	0	NULL	66.7	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of total nuclear receptors within each nuclear compartment was ( percentage of nucleoplasmic , hypertonic salt-extractable , and salt-resistant receptors ) : Cerebrum : 23.6 , 52.2 , 24.2 ; Liver : 25.2 , 57.2 , 17.5 ; Kidney : 45.9 , 33.5 , 20.6 ; Testis : 65.5 , 14.7 , 19.7 ; and Spleen : 66.7 , 18.7 , 14.6 .
	manualset3
147290	26	409613	5	NULL	NULL	0	NULL	18.7	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of total nuclear receptors within each nuclear compartment was ( percentage of nucleoplasmic , hypertonic salt-extractable , and salt-resistant receptors ) : Cerebrum : 23.6 , 52.2 , 24.2 ; Liver : 25.2 , 57.2 , 17.5 ; Kidney : 45.9 , 33.5 , 20.6 ; Testis : 65.5 , 14.7 , 19.7 ; and Spleen : 66.7 , 18.7 , 14.6 .
	manualset3
147291	27	409613	5	NULL	NULL	0	NULL	14.6	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of total nuclear receptors within each nuclear compartment was ( percentage of nucleoplasmic , hypertonic salt-extractable , and salt-resistant receptors ) : Cerebrum : 23.6 , 52.2 , 24.2 ; Liver : 25.2 , 57.2 , 17.5 ; Kidney : 45.9 , 33.5 , 20.6 ; Testis : 65.5 , 14.7 , 19.7 ; and Spleen : 66.7 , 18.7 , 14.6 .
	manualset3
147292	1	409614	5	NULL	NULL	0	NULL	distribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of various collagen types was studied in rat fibrosarcoma .
	manualset3
147293	2	409614	5	NULL	NULL	0	NULL	various collagen types	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of various collagen types was studied in rat fibrosarcoma .
	manualset3
147294	3	409614	5	NULL	NULL	0	NULL	rat fibrosarcoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of various collagen types was studied in rat fibrosarcoma .
	manualset3
147295	1	409615	5	NULL	NULL	0	NULL	disturbed export	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The disturbed export of copper into bile results in accumulation of copper in liver and secondarily in other organs such as the brain .
	manualset3
147296	2	409615	5	NULL	NULL	0	NULL	copper 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The disturbed export of copper into bile results in accumulation of copper in liver and secondarily in other organs such as the brain .
	manualset3
147297	3	409615	5	NULL	NULL	0	NULL	bile 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The disturbed export of copper into bile results in accumulation of copper in liver and secondarily in other organs such as the brain .
	manualset3
147298	4	409615	5	NULL	NULL	0	NULL	accumulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The disturbed export of copper into bile results in accumulation of copper in liver and secondarily in other organs such as the brain .
	manualset3
147299	5	409615	5	NULL	NULL	0	NULL	copper 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The disturbed export of copper into bile results in accumulation of copper in liver and secondarily in other organs such as the brain .
	manualset3
147300	6	409615	5	NULL	NULL	0	NULL	liver 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The disturbed export of copper into bile results in accumulation of copper in liver and secondarily in other organs such as the brain .
	manualset3
147301	7	409615	5	NULL	NULL	0	NULL	organs 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The disturbed export of copper into bile results in accumulation of copper in liver and secondarily in other organs such as the brain .
	manualset3
147302	8	409615	5	NULL	NULL	0	NULL	brain 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The disturbed export of copper into bile results in accumulation of copper in liver and secondarily in other organs such as the brain .
	manualset3
147303	1	409616	5	NULL	NULL	0	NULL	diuretic response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The diuretic response in normal volunteers to a new benzylamine , 2-aminomethyl-4 - ( 1 , 1-dimethylethyl ) -6 - iodophenol HCl .
	manualset3
147304	2	409616	5	NULL	NULL	0	NULL	normal volunteers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The diuretic response in normal volunteers to a new benzylamine , 2-aminomethyl-4 - ( 1 , 1-dimethylethyl ) -6 - iodophenol HCl .
	manualset3
147305	3	409616	5	NULL	NULL	0	NULL	benzylamine , 2-aminomethyl-4 - ( 1 , 1-dimethylethyl ) -6 - iodophenol HCl	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The diuretic response in normal volunteers to a new benzylamine , 2-aminomethyl-4 - ( 1 , 1-dimethylethyl ) -6 - iodophenol HCl .
	manualset3
147306	1	409617	5	NULL	NULL	0	NULL	division apparatus 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The division apparatus of plastids and mitochondria .
	manualset3
147307	2	409617	5	NULL	NULL	0	NULL	plastids 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The division apparatus of plastids and mitochondria .
	manualset3
147308	3	409617	5	NULL	NULL	0	NULL	mitochondria 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The division apparatus of plastids and mitochondria .
	manualset3
147309	1	409618	5	NULL	NULL	0	NULL	dominance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dominance of pale shades during both systole and diastole represented low-impedance , high-velocity flow within the lesion and a colored mosaic pattern representing turbulent flow was noted .
	manualset3
147310	2	409618	5	NULL	NULL	0	NULL	pale shades 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The dominance of pale shades during both systole and diastole represented low-impedance , high-velocity flow within the lesion and a colored mosaic pattern representing turbulent flow was noted .
	manualset3
147311	3	409618	5	NULL	NULL	0	NULL	systole 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The dominance of pale shades during both systole and diastole represented low-impedance , high-velocity flow within the lesion and a colored mosaic pattern representing turbulent flow was noted .
	manualset3
147312	4	409618	5	NULL	NULL	0	NULL	diastole 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The dominance of pale shades during both systole and diastole represented low-impedance , high-velocity flow within the lesion and a colored mosaic pattern representing turbulent flow was noted .
	manualset3
147313	5	409618	5	NULL	NULL	NULL	NULL	low-impedance 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The dominance of pale shades during both systole and diastole represented low-impedance , high-velocity flow within the lesion and a colored mosaic pattern representing turbulent flow was noted .
	manualset3
147314	6	409618	5	NULL	NULL	0	NULL	high-velocity flow	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dominance of pale shades during both systole and diastole represented low-impedance , high-velocity flow within the lesion and a colored mosaic pattern representing turbulent flow was noted .
	manualset3
147315	7	409618	5	NULL	NULL	0	NULL	lesion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The dominance of pale shades during both systole and diastole represented low-impedance , high-velocity flow within the lesion and a colored mosaic pattern representing turbulent flow was noted .
	manualset3
147316	8	409618	5	NULL	NULL	0	NULL	colored mosaic pattern 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The dominance of pale shades during both systole and diastole represented low-impedance , high-velocity flow within the lesion and a colored mosaic pattern representing turbulent flow was noted .
	manualset3
147317	9	409618	5	NULL	NULL	0	NULL	turbulent flow	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dominance of pale shades during both systole and diastole represented low-impedance , high-velocity flow within the lesion and a colored mosaic pattern representing turbulent flow was noted .
	manualset3
147318	1	409619	5	NULL	NULL	0	NULL	dominant effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dominant effect of artifacts , however , is bias .
	manualset3
147319	2	409619	5	NULL	NULL	0	NULL	artifacts 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The dominant effect of artifacts , however , is bias .
	manualset3
147320	1	409620	5	NULL	NULL	0	NULL	donor 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The donor was introduced by labeling either troponin C or troponin I with N - ( iodoacetyl ) - N ' - ( 5-sulfo-1-naphthyl ) ethylenediamine , while the acceptor was introduced by labeling either protein with N - ( 4 - ( dimethylamino ) phenyl-4 ' - azophenyl ) maleimide .
	manualset3
147321	2	409620	5	NULL	NULL	0	NULL	troponin C	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The donor was introduced by labeling either troponin C or troponin I with N - ( iodoacetyl ) - N ' - ( 5-sulfo-1-naphthyl ) ethylenediamine , while the acceptor was introduced by labeling either protein with N - ( 4 - ( dimethylamino ) phenyl-4 ' - azophenyl ) maleimide .
	manualset3
147322	3	409620	5	NULL	NULL	0	NULL	troponin I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The donor was introduced by labeling either troponin C or troponin I with N - ( iodoacetyl ) - N ' - ( 5-sulfo-1-naphthyl ) ethylenediamine , while the acceptor was introduced by labeling either protein with N - ( 4 - ( dimethylamino ) phenyl-4 ' - azophenyl ) maleimide .
	manualset3
147323	4	409620	5	NULL	NULL	0	NULL	N - ( iodoacetyl ) - N ' - ( 5-sulfo-1-naphthyl ) ethylenediamine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The donor was introduced by labeling either troponin C or troponin I with N - ( iodoacetyl ) - N ' - ( 5-sulfo-1-naphthyl ) ethylenediamine , while the acceptor was introduced by labeling either protein with N - ( 4 - ( dimethylamino ) phenyl-4 ' - azophenyl ) maleimide .
	manualset3
147324	5	409620	5	NULL	NULL	0	NULL	acceptor 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The donor was introduced by labeling either troponin C or troponin I with N - ( iodoacetyl ) - N ' - ( 5-sulfo-1-naphthyl ) ethylenediamine , while the acceptor was introduced by labeling either protein with N - ( 4 - ( dimethylamino ) phenyl-4 ' - azophenyl ) maleimide .
	manualset3
147325	6	409620	5	NULL	NULL	0	NULL	protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The donor was introduced by labeling either troponin C or troponin I with N - ( iodoacetyl ) - N ' - ( 5-sulfo-1-naphthyl ) ethylenediamine , while the acceptor was introduced by labeling either protein with N - ( 4 - ( dimethylamino ) phenyl-4 ' - azophenyl ) maleimide .
	manualset3
147326	7	409620	5	NULL	NULL	0	NULL	N - ( 4 - ( dimethylamino ) phenyl-4 ' - azophenyl ) maleimide	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The donor was introduced by labeling either troponin C or troponin I with N - ( iodoacetyl ) - N ' - ( 5-sulfo-1-naphthyl ) ethylenediamine , while the acceptor was introduced by labeling either protein with N - ( 4 - ( dimethylamino ) phenyl-4 ' - azophenyl ) maleimide .
	manualset3
147327	1	409621	5	NULL	NULL	0	NULL	doping mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The doping mechanism of C12A7 : Eu3 + might be attributed to Eu3 + ions substitution for two types of Ca2 + lattice sites in C12A7 .
	manualset3
147328	2	409621	5	NULL	NULL	0	NULL	C12A7 : Eu3 + 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The doping mechanism of C12A7 : Eu3 + might be attributed to Eu3 + ions substitution for two types of Ca2 + lattice sites in C12A7 .
	manualset3
147329	3	409621	5	NULL	NULL	0	NULL	Eu3 + ions substitution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The doping mechanism of C12A7 : Eu3 + might be attributed to Eu3 + ions substitution for two types of Ca2 + lattice sites in C12A7 .
	manualset3
147330	4	409621	5	NULL	NULL	0	NULL	 two types	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The doping mechanism of C12A7 : Eu3 + might be attributed to Eu3 + ions substitution for two types of Ca2 + lattice sites in C12A7 .
	manualset3
147331	5	409621	5	NULL	NULL	0	NULL	Ca2 + lattice sites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The doping mechanism of C12A7 : Eu3 + might be attributed to Eu3 + ions substitution for two types of Ca2 + lattice sites in C12A7 .
	manualset3
147332	6	409621	5	NULL	NULL	0	NULL	C12A7 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The doping mechanism of C12A7 : Eu3 + might be attributed to Eu3 + ions substitution for two types of Ca2 + lattice sites in C12A7 .
	manualset3
147333	1	409622	5	NULL	NULL	0	NULL	neuron somata	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The dorsally located neuron somata , rich in ribosomes and glycogen , are encased in multi-layered glial and fibrous sheaths .
	manualset3
147334	2	409622	5	NULL	NULL	0	NULL	ribosomes 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The dorsally located neuron somata , rich in ribosomes and glycogen , are encased in multi-layered glial and fibrous sheaths .
	manualset3
147335	3	409622	5	NULL	NULL	0	NULL	glycogen 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The dorsally located neuron somata , rich in ribosomes and glycogen , are encased in multi-layered glial and fibrous sheaths .
	manualset3
147336	4	409622	5	NULL	NULL	0	NULL	multi-layered glial sheaths	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The dorsally located neuron somata , rich in ribosomes and glycogen , are encased in multi-layered glial and fibrous sheaths .
	manualset3
147337	5	409622	5	NULL	NULL	0	NULL	fibrous sheaths	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The dorsally located neuron somata , rich in ribosomes and glycogen , are encased in multi-layered glial and fibrous sheaths .
	manualset3
147338	1	409623	5	NULL	NULL	0	NULL	dose-dependent disruptive effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose-dependent disruptive effect of acute doses of morphine on maternal behavior was more marked in the morphine-treated dams , than in the saline-treated ones , indicating a tendency for sensitisation to this effect .
	manualset3
147339	2	409623	5	NULL	NULL	0	NULL	acute doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose-dependent disruptive effect of acute doses of morphine on maternal behavior was more marked in the morphine-treated dams , than in the saline-treated ones , indicating a tendency for sensitisation to this effect .
	manualset3
147340	3	409623	5	NULL	NULL	0	NULL	morphine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose-dependent disruptive effect of acute doses of morphine on maternal behavior was more marked in the morphine-treated dams , than in the saline-treated ones , indicating a tendency for sensitisation to this effect .
	manualset3
147341	4	409623	5	NULL	NULL	0	NULL	maternal behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose-dependent disruptive effect of acute doses of morphine on maternal behavior was more marked in the morphine-treated dams , than in the saline-treated ones , indicating a tendency for sensitisation to this effect .
	manualset3
147342	5	409623	5	NULL	NULL	0	NULL	morphine-treated dams	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose-dependent disruptive effect of acute doses of morphine on maternal behavior was more marked in the morphine-treated dams , than in the saline-treated ones , indicating a tendency for sensitisation to this effect .
	manualset3
147343	6	409623	5	NULL	NULL	0	NULL	saline-treated ones	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose-dependent disruptive effect of acute doses of morphine on maternal behavior was more marked in the morphine-treated dams , than in the saline-treated ones , indicating a tendency for sensitisation to this effect .
	manualset3
147344	7	409623	5	NULL	NULL	0	NULL	sensitisation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose-dependent disruptive effect of acute doses of morphine on maternal behavior was more marked in the morphine-treated dams , than in the saline-treated ones , indicating a tendency for sensitisation to this effect .
	manualset3
147345	8	409623	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose-dependent disruptive effect of acute doses of morphine on maternal behavior was more marked in the morphine-treated dams , than in the saline-treated ones , indicating a tendency for sensitisation to this effect .
	manualset3
148675	9	409623	5	NULL	NULL	0	NULL	tendency 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose-dependent disruptive effect of acute doses of morphine on maternal behavior was more marked in the morphine-treated dams , than in the saline-treated ones , indicating a tendency for sensitisation to this effect .
	manualset3
147346	1	409624	5	NULL	NULL	0	NULL	dose-response curves	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose-response curves for tyramine were shifted to the right following treatment with dipyridamole ( 0.1-1 micro mol/L ) .
	manualset3
147347	2	409624	5	NULL	NULL	0	NULL	tyramine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose-response curves for tyramine were shifted to the right following treatment with dipyridamole ( 0.1-1 micro mol/L ) .
	manualset3
147348	3	409624	5	NULL	NULL	NULL	NULL	treatment 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The dose-response curves for tyramine were shifted to the right following treatment with dipyridamole ( 0.1-1 micro mol/L ) .
	manualset3
147349	4	409624	5	NULL	NULL	0	NULL	dipyridamole 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose-response curves for tyramine were shifted to the right following treatment with dipyridamole ( 0.1-1 micro mol/L ) .
	manualset3
147350	5	409624	5	NULL	NULL	0	NULL	0.1-1 micro mol/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose-response curves for tyramine were shifted to the right following treatment with dipyridamole ( 0.1-1 micro mol/L ) .
	manualset3
147351	1	409625	5	NULL	NULL	0	NULL	dose : response 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose : response for cardiac power from 0.1-100 nM isoproterenol was significantly shifted to the right in stunned hearts : EC50 ( nm ) increased from 0.3 + / - 0.06 to 5.2 + / - 1.86 .
	manualset3
147352	2	409625	5	NULL	NULL	0	NULL	cardiac power	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose : response for cardiac power from 0.1-100 nM isoproterenol was significantly shifted to the right in stunned hearts : EC50 ( nm ) increased from 0.3 + / - 0.06 to 5.2 + / - 1.86 .
	manualset3
147353	3	409625	5	NULL	NULL	0	NULL	 0.1-100 nM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose : response for cardiac power from 0.1-100 nM isoproterenol was significantly shifted to the right in stunned hearts : EC50 ( nm ) increased from 0.3 + / - 0.06 to 5.2 + / - 1.86 .
	manualset3
147354	4	409625	5	NULL	NULL	0	NULL	isoproterenol 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose : response for cardiac power from 0.1-100 nM isoproterenol was significantly shifted to the right in stunned hearts : EC50 ( nm ) increased from 0.3 + / - 0.06 to 5.2 + / - 1.86 .
	manualset3
147355	5	409625	5	NULL	NULL	0	NULL	stunned hearts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose : response for cardiac power from 0.1-100 nM isoproterenol was significantly shifted to the right in stunned hearts : EC50 ( nm ) increased from 0.3 + / - 0.06 to 5.2 + / - 1.86 .
	manualset3
147356	6	409625	5	NULL	NULL	0	NULL	EC50 ( nm )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose : response for cardiac power from 0.1-100 nM isoproterenol was significantly shifted to the right in stunned hearts : EC50 ( nm ) increased from 0.3 + / - 0.06 to 5.2 + / - 1.86 .
	manualset3
147357	7	409625	5	NULL	NULL	0	NULL	0.3 + / - 0.06	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose : response for cardiac power from 0.1-100 nM isoproterenol was significantly shifted to the right in stunned hearts : EC50 ( nm ) increased from 0.3 + / - 0.06 to 5.2 + / - 1.86 .
	manualset3
147358	8	409625	5	NULL	NULL	0	NULL	 5.2 + / - 1.86	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose : response for cardiac power from 0.1-100 nM isoproterenol was significantly shifted to the right in stunned hearts : EC50 ( nm ) increased from 0.3 + / - 0.06 to 5.2 + / - 1.86 .
	manualset3
147359	1	409626	5	NULL	NULL	0	NULL	dose 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose of BH4 needed to normalize liver phenylalanine hydroxylase is one eighth to one fourth that required for normal neurotransmitter metabolism in the central nervous system .
	manualset3
147360	2	409626	5	NULL	NULL	0	NULL	BH4 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose of BH4 needed to normalize liver phenylalanine hydroxylase is one eighth to one fourth that required for normal neurotransmitter metabolism in the central nervous system .
	manualset3
147361	3	409626	5	NULL	NULL	0	NULL	liver phenylalanine hydroxylase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose of BH4 needed to normalize liver phenylalanine hydroxylase is one eighth to one fourth that required for normal neurotransmitter metabolism in the central nervous system .
	manualset3
147362	4	409626	5	NULL	NULL	0	NULL	one eighth	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose of BH4 needed to normalize liver phenylalanine hydroxylase is one eighth to one fourth that required for normal neurotransmitter metabolism in the central nervous system .
	manualset3
147363	5	409626	5	NULL	NULL	NULL	NULL	one fourth	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The dose of BH4 needed to normalize liver phenylalanine hydroxylase is one eighth to one fourth that required for normal neurotransmitter metabolism in the central nervous system .
	manualset3
147364	6	409626	5	NULL	NULL	0	NULL	normal neurotransmitter metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose of BH4 needed to normalize liver phenylalanine hydroxylase is one eighth to one fourth that required for normal neurotransmitter metabolism in the central nervous system .
	manualset3
147365	7	409626	5	NULL	NULL	0	NULL	central nervous system 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose of BH4 needed to normalize liver phenylalanine hydroxylase is one eighth to one fourth that required for normal neurotransmitter metabolism in the central nervous system .
	manualset3
147366	1	409627	5	NULL	NULL	0	NULL	dose point kernel method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose point kernel method , which takes into account absorption in the strut material ( = self-absorption ) , was based on different beta-emitting point source distributions in water by itself and surrounded by steel spheres of different thicknesses .
	manualset3
147367	2	409627	5	NULL	NULL	0	NULL	account 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose point kernel method , which takes into account absorption in the strut material ( = self-absorption ) , was based on different beta-emitting point source distributions in water by itself and surrounded by steel spheres of different thicknesses .
	manualset3
147368	3	409627	5	NULL	NULL	0	NULL	absorption 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose point kernel method , which takes into account absorption in the strut material ( = self-absorption ) , was based on different beta-emitting point source distributions in water by itself and surrounded by steel spheres of different thicknesses .
	manualset3
147369	4	409627	5	NULL	NULL	0	NULL	strut material 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose point kernel method , which takes into account absorption in the strut material ( = self-absorption ) , was based on different beta-emitting point source distributions in water by itself and surrounded by steel spheres of different thicknesses .
	manualset3
147370	5	409627	5	NULL	NULL	0	NULL	self-absorption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose point kernel method , which takes into account absorption in the strut material ( = self-absorption ) , was based on different beta-emitting point source distributions in water by itself and surrounded by steel spheres of different thicknesses .
	manualset3
147371	6	409627	5	NULL	NULL	0	NULL	 beta-emitting point source distributions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose point kernel method , which takes into account absorption in the strut material ( = self-absorption ) , was based on different beta-emitting point source distributions in water by itself and surrounded by steel spheres of different thicknesses .
	manualset3
147372	7	409627	5	NULL	NULL	0	NULL	water 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose point kernel method , which takes into account absorption in the strut material ( = self-absorption ) , was based on different beta-emitting point source distributions in water by itself and surrounded by steel spheres of different thicknesses .
	manualset3
147373	8	409627	5	NULL	NULL	0	NULL	steel spheres	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose point kernel method , which takes into account absorption in the strut material ( = self-absorption ) , was based on different beta-emitting point source distributions in water by itself and surrounded by steel spheres of different thicknesses .
	manualset3
147374	9	409627	5	NULL	NULL	0	NULL	thicknesses 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose point kernel method , which takes into account absorption in the strut material ( = self-absorption ) , was based on different beta-emitting point source distributions in water by itself and surrounded by steel spheres of different thicknesses .
	manualset3
147375	1	409628	5	NULL	NULL	0	NULL	dose response 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose response obtained in this study is lower than the linear component of the dose response for stable chromosome aberrations obtained for the Japanese atomic bomb survivors .
	manualset3
147376	2	409628	5	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose response obtained in this study is lower than the linear component of the dose response for stable chromosome aberrations obtained for the Japanese atomic bomb survivors .
	manualset3
147377	3	409628	5	NULL	NULL	0	NULL	linear component 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose response obtained in this study is lower than the linear component of the dose response for stable chromosome aberrations obtained for the Japanese atomic bomb survivors .
	manualset3
147378	4	409628	5	NULL	NULL	0	NULL	dose response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose response obtained in this study is lower than the linear component of the dose response for stable chromosome aberrations obtained for the Japanese atomic bomb survivors .
	manualset3
147379	5	409628	5	NULL	NULL	0	NULL	stable chromosome aberrations 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose response obtained in this study is lower than the linear component of the dose response for stable chromosome aberrations obtained for the Japanese atomic bomb survivors .
	manualset3
147380	6	409628	5	NULL	NULL	0	NULL	Japanese atomic bomb survivors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The dose response obtained in this study is lower than the linear component of the dose response for stable chromosome aberrations obtained for the Japanese atomic bomb survivors .
	manualset3
147381	1	409629	5	NULL	NULL	0	NULL	doses 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The doses of Cd from 0.1 to 1 mg Cd g ( -1 ) did not influence ovarian development .
	manualset3
147382	2	409629	5	NULL	NULL	0	NULL	Cd 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The doses of Cd from 0.1 to 1 mg Cd g ( -1 ) did not influence ovarian development .
	manualset3
147383	3	409629	5	NULL	NULL	NULL	NULL	 0.1 to 1 mg Cd g ( -1 )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The doses of Cd from 0.1 to 1 mg Cd g ( -1 ) did not influence ovarian development .
	manualset3
147384	4	409629	5	NULL	NULL	NULL	NULL	influence 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The doses of Cd from 0.1 to 1 mg Cd g ( -1 ) did not influence ovarian development .
	manualset3
147385	5	409629	5	NULL	NULL	NULL	NULL	ovarian development 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The doses of Cd from 0.1 to 1 mg Cd g ( -1 ) did not influence ovarian development .
	manualset3
147386	1	409630	5	NULL	NULL	0	NULL	double logarithm plots	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The double logarithm plots of pseudo-first order rate constant versus reagent concentrations gave slopes of 0.88 ( PGO ) and 0.90 ( BD ) , respectively , suggesting that the inactivation may possibly result from reaction of at least one arginyl residue at the active site of H ( + ) - translocating PPase .
	manualset3
147387	2	409630	5	NULL	NULL	0	NULL	pseudo-first order rate constant	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The double logarithm plots of pseudo-first order rate constant versus reagent concentrations gave slopes of 0.88 ( PGO ) and 0.90 ( BD ) , respectively , suggesting that the inactivation may possibly result from reaction of at least one arginyl residue at the active site of H ( + ) - translocating PPase .
	manualset3
147388	3	409630	5	NULL	NULL	0	NULL	reagent concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The double logarithm plots of pseudo-first order rate constant versus reagent concentrations gave slopes of 0.88 ( PGO ) and 0.90 ( BD ) , respectively , suggesting that the inactivation may possibly result from reaction of at least one arginyl residue at the active site of H ( + ) - translocating PPase .
	manualset3
147389	4	409630	5	NULL	NULL	0	NULL	slopes 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The double logarithm plots of pseudo-first order rate constant versus reagent concentrations gave slopes of 0.88 ( PGO ) and 0.90 ( BD ) , respectively , suggesting that the inactivation may possibly result from reaction of at least one arginyl residue at the active site of H ( + ) - translocating PPase .
	manualset3
147390	5	409630	5	NULL	NULL	0	NULL	0.88 ( PGO )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The double logarithm plots of pseudo-first order rate constant versus reagent concentrations gave slopes of 0.88 ( PGO ) and 0.90 ( BD ) , respectively , suggesting that the inactivation may possibly result from reaction of at least one arginyl residue at the active site of H ( + ) - translocating PPase .
	manualset3
147391	6	409630	5	NULL	NULL	0	NULL	0.90 ( BD )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The double logarithm plots of pseudo-first order rate constant versus reagent concentrations gave slopes of 0.88 ( PGO ) and 0.90 ( BD ) , respectively , suggesting that the inactivation may possibly result from reaction of at least one arginyl residue at the active site of H ( + ) - translocating PPase .
	manualset3
147392	7	409630	5	NULL	NULL	0	NULL	inactivation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The double logarithm plots of pseudo-first order rate constant versus reagent concentrations gave slopes of 0.88 ( PGO ) and 0.90 ( BD ) , respectively , suggesting that the inactivation may possibly result from reaction of at least one arginyl residue at the active site of H ( + ) - translocating PPase .
	manualset3
147393	8	409630	5	NULL	NULL	0	NULL	result 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The double logarithm plots of pseudo-first order rate constant versus reagent concentrations gave slopes of 0.88 ( PGO ) and 0.90 ( BD ) , respectively , suggesting that the inactivation may possibly result from reaction of at least one arginyl residue at the active site of H ( + ) - translocating PPase .
	manualset3
147394	9	409630	5	NULL	NULL	0	NULL	reaction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The double logarithm plots of pseudo-first order rate constant versus reagent concentrations gave slopes of 0.88 ( PGO ) and 0.90 ( BD ) , respectively , suggesting that the inactivation may possibly result from reaction of at least one arginyl residue at the active site of H ( + ) - translocating PPase .
	manualset3
147395	10	409630	5	NULL	NULL	0	NULL	one	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The double logarithm plots of pseudo-first order rate constant versus reagent concentrations gave slopes of 0.88 ( PGO ) and 0.90 ( BD ) , respectively , suggesting that the inactivation may possibly result from reaction of at least one arginyl residue at the active site of H ( + ) - translocating PPase .
	manualset3
147396	11	409630	5	NULL	NULL	0	NULL	arginyl residue 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The double logarithm plots of pseudo-first order rate constant versus reagent concentrations gave slopes of 0.88 ( PGO ) and 0.90 ( BD ) , respectively , suggesting that the inactivation may possibly result from reaction of at least one arginyl residue at the active site of H ( + ) - translocating PPase .
	manualset3
147397	12	409630	5	NULL	NULL	0	NULL	 active site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The double logarithm plots of pseudo-first order rate constant versus reagent concentrations gave slopes of 0.88 ( PGO ) and 0.90 ( BD ) , respectively , suggesting that the inactivation may possibly result from reaction of at least one arginyl residue at the active site of H ( + ) - translocating PPase .
	manualset3
147398	13	409630	5	NULL	NULL	0	NULL	H ( + ) - translocating PPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The double logarithm plots of pseudo-first order rate constant versus reagent concentrations gave slopes of 0.88 ( PGO ) and 0.90 ( BD ) , respectively , suggesting that the inactivation may possibly result from reaction of at least one arginyl residue at the active site of H ( + ) - translocating PPase .
	manualset3
147399	1	409631	5	NULL	NULL	0	NULL	smaller gap clearance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A smaller gap clearance will also increase the flow resistance and hence , decrease the nondimensional leakage flow rate .
	manualset3
147400	2	409631	5	NULL	NULL	NULL	NULL	flow resistance	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A smaller gap clearance will also increase the flow resistance and hence , decrease the nondimensional leakage flow rate .
	manualset3
147401	3	409631	5	NULL	NULL	0	NULL	nondimensional leakage flow rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A smaller gap clearance will also increase the flow resistance and hence , decrease the nondimensional leakage flow rate .
	manualset3
147402	1	409632	5	NULL	NULL	0	NULL	downfield shift 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The downfield shift of H-2 of galactose residue demonstrated the presence of 2-O-sulfonate group .
	manualset3
147403	2	409632	5	NULL	NULL	0	NULL	H-2	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The downfield shift of H-2 of galactose residue demonstrated the presence of 2-O-sulfonate group .
	manualset3
147404	3	409632	5	NULL	NULL	0	NULL	galactose residue	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The downfield shift of H-2 of galactose residue demonstrated the presence of 2-O-sulfonate group .
	manualset3
147405	4	409632	5	NULL	NULL	0	NULL	2-O-sulfonate group 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The downfield shift of H-2 of galactose residue demonstrated the presence of 2-O-sulfonate group .
	manualset3
147406	1	409633	5	NULL	NULL	0	NULL	clinical features	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The dramatic clinical and pathological features of this case are compared with those of the nine previously reported cases of infection due to Capnocytophaga species occurring in pregnancy .
	manualset3
147407	2	409633	5	NULL	NULL	0	NULL	pathological features	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The dramatic clinical and pathological features of this case are compared with those of the nine previously reported cases of infection due to Capnocytophaga species occurring in pregnancy .
	manualset3
147408	3	409633	5	NULL	NULL	0	NULL	case 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The dramatic clinical and pathological features of this case are compared with those of the nine previously reported cases of infection due to Capnocytophaga species occurring in pregnancy .
	manualset3
147409	4	409633	5	NULL	NULL	0	NULL	nine 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The dramatic clinical and pathological features of this case are compared with those of the nine previously reported cases of infection due to Capnocytophaga species occurring in pregnancy .
	manualset3
147410	5	409633	5	NULL	NULL	0	NULL	cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The dramatic clinical and pathological features of this case are compared with those of the nine previously reported cases of infection due to Capnocytophaga species occurring in pregnancy .
	manualset3
147411	6	409633	5	NULL	NULL	0	NULL	infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The dramatic clinical and pathological features of this case are compared with those of the nine previously reported cases of infection due to Capnocytophaga species occurring in pregnancy .
	manualset3
147412	7	409633	5	NULL	NULL	0	NULL	Capnocytophaga species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The dramatic clinical and pathological features of this case are compared with those of the nine previously reported cases of infection due to Capnocytophaga species occurring in pregnancy .
	manualset3
147413	8	409633	5	NULL	NULL	0	NULL	pregnancy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The dramatic clinical and pathological features of this case are compared with those of the nine previously reported cases of infection due to Capnocytophaga species occurring in pregnancy .
	manualset3
147414	1	409634	5	NULL	NULL	0	NULL	dramatic rise 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dramatic rise in gestational diabetes and type 2 diabetes in the young may therefore be traced to food patterns that exaggerate postprandial glycemia and insulinemia .
	manualset3
147415	2	409634	5	NULL	NULL	0	NULL	gestational diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The dramatic rise in gestational diabetes and type 2 diabetes in the young may therefore be traced to food patterns that exaggerate postprandial glycemia and insulinemia .
	manualset3
147416	3	409634	5	NULL	NULL	0	NULL	type 2 diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The dramatic rise in gestational diabetes and type 2 diabetes in the young may therefore be traced to food patterns that exaggerate postprandial glycemia and insulinemia .
	manualset3
147417	4	409634	5	NULL	NULL	0	NULL	young 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The dramatic rise in gestational diabetes and type 2 diabetes in the young may therefore be traced to food patterns that exaggerate postprandial glycemia and insulinemia .
	manualset3
147418	5	409634	5	NULL	NULL	0	NULL	food patterns	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The dramatic rise in gestational diabetes and type 2 diabetes in the young may therefore be traced to food patterns that exaggerate postprandial glycemia and insulinemia .
	manualset3
147419	6	409634	5	NULL	NULL	0	NULL	postprandial glycemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The dramatic rise in gestational diabetes and type 2 diabetes in the young may therefore be traced to food patterns that exaggerate postprandial glycemia and insulinemia .
	manualset3
147420	7	409634	5	NULL	NULL	0	NULL	insulinemia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The dramatic rise in gestational diabetes and type 2 diabetes in the young may therefore be traced to food patterns that exaggerate postprandial glycemia and insulinemia .
	manualset3
147421	1	409635	5	NULL	NULL	0	NULL	drawer test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The drawer test , the pivot shift and the thigh muscle stretching tests showed greater mobility among carpet and floor layers than among painters .
	manualset3
147422	2	409635	5	NULL	NULL	0	NULL	pivot shift test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The drawer test , the pivot shift and the thigh muscle stretching tests showed greater mobility among carpet and floor layers than among painters .
	manualset3
147423	3	409635	5	NULL	NULL	0	NULL	thigh muscle stretching tests	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The drawer test , the pivot shift and the thigh muscle stretching tests showed greater mobility among carpet and floor layers than among painters .
	manualset3
147424	4	409635	5	NULL	NULL	0	NULL	mobility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The drawer test , the pivot shift and the thigh muscle stretching tests showed greater mobility among carpet and floor layers than among painters .
	manualset3
147425	5	409635	5	NULL	NULL	0	NULL	carpet 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The drawer test , the pivot shift and the thigh muscle stretching tests showed greater mobility among carpet and floor layers than among painters .
	manualset3
147426	6	409635	5	NULL	NULL	0	NULL	floor layers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The drawer test , the pivot shift and the thigh muscle stretching tests showed greater mobility among carpet and floor layers than among painters .
	manualset3
147427	7	409635	5	NULL	NULL	0	NULL	painters 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The drawer test , the pivot shift and the thigh muscle stretching tests showed greater mobility among carpet and floor layers than among painters .
	manualset3
147428	1	409636	5	NULL	NULL	0	NULL	drinking water	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The drinking water and ambient air in vicinity of the works were found to be polluted by toxic substances .
	manualset3
147429	2	409636	5	NULL	NULL	0	NULL	ambient air	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The drinking water and ambient air in vicinity of the works were found to be polluted by toxic substances .
	manualset3
147430	3	409636	5	NULL	NULL	0	NULL	vicinity 	n												NULL		0	NULL	NULL	NULL	NULL	NULL	The drinking water and ambient air in vicinity of the works were found to be polluted by toxic substances .
	manualset3
147431	4	409636	5	NULL	NULL	0	NULL	toxic substances	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The drinking water and ambient air in vicinity of the works were found to be polluted by toxic substances .
	manualset3
147432	1	409637	5	NULL	NULL	0	NULL	driving forces 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The driving forces are the commercial and military applications for detectors , and with few exceptions there has not been sufficient funding available to mount a detector development program for astronomy .
	manualset3
147433	2	409637	5	NULL	NULL	0	NULL	commercial applications 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The driving forces are the commercial and military applications for detectors , and with few exceptions there has not been sufficient funding available to mount a detector development program for astronomy .
	manualset3
147434	3	409637	5	NULL	NULL	0	NULL	military applications 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The driving forces are the commercial and military applications for detectors , and with few exceptions there has not been sufficient funding available to mount a detector development program for astronomy .
	manualset3
147435	4	409637	5	NULL	NULL	0	NULL	detectors 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The driving forces are the commercial and military applications for detectors , and with few exceptions there has not been sufficient funding available to mount a detector development program for astronomy .
	manualset3
147436	5	409637	5	NULL	NULL	0	NULL	exceptions 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The driving forces are the commercial and military applications for detectors , and with few exceptions there has not been sufficient funding available to mount a detector development program for astronomy .
	manualset3
147437	6	409637	5	NULL	NULL	0	NULL	detector development program	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The driving forces are the commercial and military applications for detectors , and with few exceptions there has not been sufficient funding available to mount a detector development program for astronomy .
	manualset3
147438	7	409637	5	NULL	NULL	0	NULL	astronomy 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The driving forces are the commercial and military applications for detectors , and with few exceptions there has not been sufficient funding available to mount a detector development program for astronomy .
	manualset3
147439	1	409638	5	NULL	NULL	0	NULL	drug 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The drug caused a significant reduction of post-operative pain , swelling and trismus .
	manualset3
147440	2	409638	5	NULL	NULL	0	NULL	reduction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The drug caused a significant reduction of post-operative pain , swelling and trismus .
	manualset3
147441	3	409638	5	NULL	NULL	0	NULL	post-operative pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The drug caused a significant reduction of post-operative pain , swelling and trismus .
	manualset3
147442	4	409638	5	NULL	NULL	0	NULL	swelling 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The drug caused a significant reduction of post-operative pain , swelling and trismus .
	manualset3
147443	5	409638	5	NULL	NULL	0	NULL	trismus 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The drug caused a significant reduction of post-operative pain , swelling and trismus .
	manualset3
147444	1	409639	5	NULL	NULL	0	NULL	drug loading	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The drug loading was confirmed by the decrease of specific surface area and pore volume between MCM-41 and the inclusion compound .
	manualset3
147445	2	409639	5	NULL	NULL	0	NULL	specific surface area 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The drug loading was confirmed by the decrease of specific surface area and pore volume between MCM-41 and the inclusion compound .
	manualset3
147446	3	409639	5	NULL	NULL	0	NULL	pore volume 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The drug loading was confirmed by the decrease of specific surface area and pore volume between MCM-41 and the inclusion compound .
	manualset3
147447	4	409639	5	NULL	NULL	0	NULL	MCM-41 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The drug loading was confirmed by the decrease of specific surface area and pore volume between MCM-41 and the inclusion compound .
	manualset3
147448	5	409639	5	NULL	NULL	0	NULL	inclusion compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The drug loading was confirmed by the decrease of specific surface area and pore volume between MCM-41 and the inclusion compound .
	manualset3
147449	1	409640	5	NULL	NULL	0	NULL	drug susceptibility	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The drug susceptibility of Staphylococcus aureus strains isolated from nose and pharynx .
	manualset3
147450	2	409640	5	NULL	NULL	0	NULL	Staphylococcus aureus strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The drug susceptibility of Staphylococcus aureus strains isolated from nose and pharynx .
	manualset3
147451	3	409640	5	NULL	NULL	0	NULL	nose 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The drug susceptibility of Staphylococcus aureus strains isolated from nose and pharynx .
	manualset3
147452	4	409640	5	NULL	NULL	0	NULL	pharynx 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The drug susceptibility of Staphylococcus aureus strains isolated from nose and pharynx .
	manualset3
147453	1	409641	5	NULL	NULL	0	NULL	solid-state nitric oxide ( NO ) sensor 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	A solid-state nitric oxide ( NO ) sensor for asthma monitoring has been identified , and efforts are underway to miniaturize this NO sensor technology and integrate it into a smart sensor system .
	manualset3
147454	2	409641	5	NULL	NULL	0	NULL	asthma monitoring	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A solid-state nitric oxide ( NO ) sensor for asthma monitoring has been identified , and efforts are underway to miniaturize this NO sensor technology and integrate it into a smart sensor system .
	manualset3
147455	3	409641	5	NULL	NULL	0	NULL	efforts 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A solid-state nitric oxide ( NO ) sensor for asthma monitoring has been identified , and efforts are underway to miniaturize this NO sensor technology and integrate it into a smart sensor system .
	manualset3
147456	4	409641	5	NULL	NULL	0	NULL	NO sensor technology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A solid-state nitric oxide ( NO ) sensor for asthma monitoring has been identified , and efforts are underway to miniaturize this NO sensor technology and integrate it into a smart sensor system .
	manualset3
147457	5	409641	5	NULL	NULL	0	NULL	smart sensor system	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A solid-state nitric oxide ( NO ) sensor for asthma monitoring has been identified , and efforts are underway to miniaturize this NO sensor technology and integrate it into a smart sensor system .
	manualset3
147458	1	409642	5	NULL	NULL	0	NULL	dtdS gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The dtdS gene encodes a 292 amino acid polypeptide .
	manualset3
147459	2	409642	5	NULL	NULL	0	NULL	292 amino acid polypeptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The dtdS gene encodes a 292 amino acid polypeptide .
	manualset3
147460	1	409643	5	NULL	NULL	0	NULL	dual specificity protein kinase CLK3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The dual specificity protein kinase CLK3 is abundantly expressed in mature mouse spermatozoa .
	manualset3
147461	2	409643	5	NULL	NULL	0	NULL	mature mouse spermatozoa 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The dual specificity protein kinase CLK3 is abundantly expressed in mature mouse spermatozoa .
	manualset3
147462	1	409644	5	NULL	NULL	0	NULL	ductus venosus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The ductus venosus has an important role in the regulation of nutrient partitioning in the fetus .
	manualset3
147463	2	409644	5	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ductus venosus has an important role in the regulation of nutrient partitioning in the fetus .
	manualset3
147464	3	409644	5	NULL	NULL	0	NULL	regulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ductus venosus has an important role in the regulation of nutrient partitioning in the fetus .
	manualset3
147465	4	409644	5	NULL	NULL	0	NULL	nutrient partitioning	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ductus venosus has an important role in the regulation of nutrient partitioning in the fetus .
	manualset3
147466	5	409644	5	NULL	NULL	0	NULL	fetus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The ductus venosus has an important role in the regulation of nutrient partitioning in the fetus .
	manualset3
147467	1	409645	5	NULL	NULL	0	NULL	duration 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration ( 2.5 to 7.5 min ) and the pH ( 10.5 to 12.5 ) of the cyanogen bromide activation of microcristalline cellulose did not affect the coupling capacity or the immunoreactivity of the second antibody , nor did it augment aspecific adsorption of free gonadotrophin on the cellulose matrix .
	manualset3
147468	2	409645	5	NULL	NULL	0	NULL	2.5 to 7.5 min 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration ( 2.5 to 7.5 min ) and the pH ( 10.5 to 12.5 ) of the cyanogen bromide activation of microcristalline cellulose did not affect the coupling capacity or the immunoreactivity of the second antibody , nor did it augment aspecific adsorption of free gonadotrophin on the cellulose matrix .
	manualset3
147469	3	409645	5	NULL	NULL	0	NULL	pH 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration ( 2.5 to 7.5 min ) and the pH ( 10.5 to 12.5 ) of the cyanogen bromide activation of microcristalline cellulose did not affect the coupling capacity or the immunoreactivity of the second antibody , nor did it augment aspecific adsorption of free gonadotrophin on the cellulose matrix .
	manualset3
147470	4	409645	5	NULL	NULL	0	NULL	10.5 to 12.5	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration ( 2.5 to 7.5 min ) and the pH ( 10.5 to 12.5 ) of the cyanogen bromide activation of microcristalline cellulose did not affect the coupling capacity or the immunoreactivity of the second antibody , nor did it augment aspecific adsorption of free gonadotrophin on the cellulose matrix .
	manualset3
147471	5	409645	5	NULL	NULL	0	NULL	cyanogen bromide activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration ( 2.5 to 7.5 min ) and the pH ( 10.5 to 12.5 ) of the cyanogen bromide activation of microcristalline cellulose did not affect the coupling capacity or the immunoreactivity of the second antibody , nor did it augment aspecific adsorption of free gonadotrophin on the cellulose matrix .
	manualset3
147472	6	409645	5	NULL	NULL	0	NULL	microcristalline cellulose	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration ( 2.5 to 7.5 min ) and the pH ( 10.5 to 12.5 ) of the cyanogen bromide activation of microcristalline cellulose did not affect the coupling capacity or the immunoreactivity of the second antibody , nor did it augment aspecific adsorption of free gonadotrophin on the cellulose matrix .
	manualset3
147474	8	409645	5	NULL	NULL	0	NULL	coupling capacity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration ( 2.5 to 7.5 min ) and the pH ( 10.5 to 12.5 ) of the cyanogen bromide activation of microcristalline cellulose did not affect the coupling capacity or the immunoreactivity of the second antibody , nor did it augment aspecific adsorption of free gonadotrophin on the cellulose matrix .
	manualset3
147475	9	409645	5	NULL	NULL	0	NULL	immunoreactivity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration ( 2.5 to 7.5 min ) and the pH ( 10.5 to 12.5 ) of the cyanogen bromide activation of microcristalline cellulose did not affect the coupling capacity or the immunoreactivity of the second antibody , nor did it augment aspecific adsorption of free gonadotrophin on the cellulose matrix .
	manualset3
147476	10	409645	5	NULL	NULL	0	NULL	second antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration ( 2.5 to 7.5 min ) and the pH ( 10.5 to 12.5 ) of the cyanogen bromide activation of microcristalline cellulose did not affect the coupling capacity or the immunoreactivity of the second antibody , nor did it augment aspecific adsorption of free gonadotrophin on the cellulose matrix .
	manualset3
147477	11	409645	5	NULL	NULL	0	NULL	aspecific adsorption	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration ( 2.5 to 7.5 min ) and the pH ( 10.5 to 12.5 ) of the cyanogen bromide activation of microcristalline cellulose did not affect the coupling capacity or the immunoreactivity of the second antibody , nor did it augment aspecific adsorption of free gonadotrophin on the cellulose matrix .
	manualset3
147478	12	409645	5	NULL	NULL	0	NULL	free gonadotrophin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration ( 2.5 to 7.5 min ) and the pH ( 10.5 to 12.5 ) of the cyanogen bromide activation of microcristalline cellulose did not affect the coupling capacity or the immunoreactivity of the second antibody , nor did it augment aspecific adsorption of free gonadotrophin on the cellulose matrix .
	manualset3
147479	13	409645	5	NULL	NULL	0	NULL	cellulose matrix	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration ( 2.5 to 7.5 min ) and the pH ( 10.5 to 12.5 ) of the cyanogen bromide activation of microcristalline cellulose did not affect the coupling capacity or the immunoreactivity of the second antibody , nor did it augment aspecific adsorption of free gonadotrophin on the cellulose matrix .
	manualset3
147480	1	409646	5	NULL	NULL	0	NULL	duration 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration of cardiac asystole induced by ocular compression was measured in 100 consecutive children referred for electroencephalographic examination after one or more febrile convulsions ( FC ) .
	manualset3
147481	2	409646	5	NULL	NULL	0	NULL	cardiac asystole 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration of cardiac asystole induced by ocular compression was measured in 100 consecutive children referred for electroencephalographic examination after one or more febrile convulsions ( FC ) .
	manualset3
147482	3	409646	5	NULL	NULL	0	NULL	ocular compression 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration of cardiac asystole induced by ocular compression was measured in 100 consecutive children referred for electroencephalographic examination after one or more febrile convulsions ( FC ) .
	manualset3
147483	4	409646	5	NULL	NULL	0	NULL	100 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration of cardiac asystole induced by ocular compression was measured in 100 consecutive children referred for electroencephalographic examination after one or more febrile convulsions ( FC ) .
	manualset3
147484	5	409646	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration of cardiac asystole induced by ocular compression was measured in 100 consecutive children referred for electroencephalographic examination after one or more febrile convulsions ( FC ) .
	manualset3
147485	6	409646	5	NULL	NULL	0	NULL	electroencephalographic examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration of cardiac asystole induced by ocular compression was measured in 100 consecutive children referred for electroencephalographic examination after one or more febrile convulsions ( FC ) .
	manualset3
147486	7	409646	5	NULL	NULL	0	NULL	one or more 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration of cardiac asystole induced by ocular compression was measured in 100 consecutive children referred for electroencephalographic examination after one or more febrile convulsions ( FC ) .
	manualset3
147487	8	409646	5	NULL	NULL	0	NULL	febrile convulsions ( FC ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration of cardiac asystole induced by ocular compression was measured in 100 consecutive children referred for electroencephalographic examination after one or more febrile convulsions ( FC ) .
	manualset3
147488	1	409647	5	NULL	NULL	0	NULL	duration 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration of dialysis session was 220 + / - 24 minutes , with a rate of blood flow 297 + / - 47 ml/min .
	manualset3
147489	2	409647	5	NULL	NULL	0	NULL	dialysis session	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration of dialysis session was 220 + / - 24 minutes , with a rate of blood flow 297 + / - 47 ml/min .
	manualset3
147490	3	409647	5	NULL	NULL	0	NULL	220 + / - 24 minutes	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration of dialysis session was 220 + / - 24 minutes , with a rate of blood flow 297 + / - 47 ml/min .
	manualset3
147491	4	409647	5	NULL	NULL	0	NULL	rate of blood flow	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration of dialysis session was 220 + / - 24 minutes , with a rate of blood flow 297 + / - 47 ml/min .
	manualset3
147492	5	409647	5	NULL	NULL	0	NULL	297 + / - 47 ml/min	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration of dialysis session was 220 + / - 24 minutes , with a rate of blood flow 297 + / - 47 ml/min .
	manualset3
147493	1	409648	5	NULL	NULL	0	NULL	duration 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration of hospitalization was shown to depend not only on the clinical characteristics of the patient but also on his or her personality and socio-psychological characteristics both in the process of illness and in the premorbid state .
	manualset3
147494	2	409648	5	NULL	NULL	0	NULL	hospitalization 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration of hospitalization was shown to depend not only on the clinical characteristics of the patient but also on his or her personality and socio-psychological characteristics both in the process of illness and in the premorbid state .
	manualset3
147495	3	409648	5	NULL	NULL	0	NULL	clinical characteristics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration of hospitalization was shown to depend not only on the clinical characteristics of the patient but also on his or her personality and socio-psychological characteristics both in the process of illness and in the premorbid state .
	manualset3
147496	4	409648	5	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration of hospitalization was shown to depend not only on the clinical characteristics of the patient but also on his or her personality and socio-psychological characteristics both in the process of illness and in the premorbid state .
	manualset3
147497	5	409648	5	NULL	NULL	0	NULL	personality 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration of hospitalization was shown to depend not only on the clinical characteristics of the patient but also on his or her personality and socio-psychological characteristics both in the process of illness and in the premorbid state .
	manualset3
147498	6	409648	5	NULL	NULL	0	NULL	socio-psychological characteristics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration of hospitalization was shown to depend not only on the clinical characteristics of the patient but also on his or her personality and socio-psychological characteristics both in the process of illness and in the premorbid state .
	manualset3
147499	7	409648	5	NULL	NULL	0	NULL	illness 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration of hospitalization was shown to depend not only on the clinical characteristics of the patient but also on his or her personality and socio-psychological characteristics both in the process of illness and in the premorbid state .
	manualset3
147500	8	409648	5	NULL	NULL	0	NULL	premorbid state	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration of hospitalization was shown to depend not only on the clinical characteristics of the patient but also on his or her personality and socio-psychological characteristics both in the process of illness and in the premorbid state .
	manualset3
147501	1	409649	5	NULL	NULL	0	NULL	duration 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration of the examination was higher with the robot ( 16 + / - 10 min ) than for the reference echography ( 11 + / - 4 min = or ) +43 % with the robot compare to reference echography .
	manualset3
147502	2	409649	5	NULL	NULL	0	NULL	examination 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration of the examination was higher with the robot ( 16 + / - 10 min ) than for the reference echography ( 11 + / - 4 min = or ) +43 % with the robot compare to reference echography .
	manualset3
147503	3	409649	5	NULL	NULL	0	NULL	robot 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration of the examination was higher with the robot ( 16 + / - 10 min ) than for the reference echography ( 11 + / - 4 min = or ) +43 % with the robot compare to reference echography .
	manualset3
147504	4	409649	5	NULL	NULL	0	NULL	 16 + / - 10 min 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration of the examination was higher with the robot ( 16 + / - 10 min ) than for the reference echography ( 11 + / - 4 min = or ) +43 % with the robot compare to reference echography .
	manualset3
147505	5	409649	5	NULL	NULL	0	NULL	reference echography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration of the examination was higher with the robot ( 16 + / - 10 min ) than for the reference echography ( 11 + / - 4 min = or ) +43 % with the robot compare to reference echography .
	manualset3
147506	6	409649	5	NULL	NULL	NULL	NULL	 ( 11 + / - 4 min = or ) +43 %	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The duration of the examination was higher with the robot ( 16 + / - 10 min ) than for the reference echography ( 11 + / - 4 min = or ) +43 % with the robot compare to reference echography .
	manualset3
147507	7	409649	5	NULL	NULL	0	NULL	robot 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration of the examination was higher with the robot ( 16 + / - 10 min ) than for the reference echography ( 11 + / - 4 min = or ) +43 % with the robot compare to reference echography .
	manualset3
147508	8	409649	5	NULL	NULL	0	NULL	reference echography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The duration of the examination was higher with the robot ( 16 + / - 10 min ) than for the reference echography ( 11 + / - 4 min = or ) +43 % with the robot compare to reference echography .
	manualset3
147509	1	409650	5	NULL	NULL	0	NULL	special strategy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A special strategy was used for the construction of strains with a disrupted copy of murI , because of a limited capability of E. coli strains grown in rich medium to internalize D-glutamic acid .
	manualset3
147510	2	409650	5	NULL	NULL	0	NULL	construction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A special strategy was used for the construction of strains with a disrupted copy of murI , because of a limited capability of E. coli strains grown in rich medium to internalize D-glutamic acid .
	manualset3
147512	4	409650	5	NULL	NULL	0	NULL	strains 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A special strategy was used for the construction of strains with a disrupted copy of murI , because of a limited capability of E. coli strains grown in rich medium to internalize D-glutamic acid .
	manualset3
147513	5	409650	5	NULL	NULL	0	NULL	disrupted copy of murI 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A special strategy was used for the construction of strains with a disrupted copy of murI , because of a limited capability of E. coli strains grown in rich medium to internalize D-glutamic acid .
	manualset3
147514	6	409650	5	NULL	NULL	0	NULL	limited capability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A special strategy was used for the construction of strains with a disrupted copy of murI , because of a limited capability of E. coli strains grown in rich medium to internalize D-glutamic acid .
	manualset3
147515	7	409650	5	NULL	NULL	0	NULL	limited capability	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A special strategy was used for the construction of strains with a disrupted copy of murI , because of a limited capability of E. coli strains grown in rich medium to internalize D-glutamic acid .
	manualset3
147516	8	409650	5	NULL	NULL	0	NULL	rich medium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A special strategy was used for the construction of strains with a disrupted copy of murI , because of a limited capability of E. coli strains grown in rich medium to internalize D-glutamic acid .
	manualset3
147517	9	409650	5	NULL	NULL	0	NULL	D-glutamic acid 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A special strategy was used for the construction of strains with a disrupted copy of murI , because of a limited capability of E. coli strains grown in rich medium to internalize D-glutamic acid .
	manualset3
147518	1	409651	5	NULL	NULL	0	NULL	duty 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The duty to attend upon the sick .
	manualset3
147519	2	409651	5	NULL	NULL	0	NULL	sick 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The duty to attend upon the sick .
	manualset3
147520	1	409652	5	NULL	NULL	0	NULL	dynamic interplay	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamic interplay between static and sliding friction is fundamental to many animal movements .
	manualset3
147521	2	409652	5	NULL	NULL	0	NULL	static friction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamic interplay between static and sliding friction is fundamental to many animal movements .
	manualset3
147522	3	409652	5	NULL	NULL	0	NULL	sliding friction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamic interplay between static and sliding friction is fundamental to many animal movements .
	manualset3
147523	4	409652	5	NULL	NULL	0	NULL	animal movements 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamic interplay between static and sliding friction is fundamental to many animal movements .
	manualset3
147524	1	409653	5	NULL	NULL	0	NULL	dynamics 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamics of cytochrome P450 CYP1A1/2 activity in the course of spheroid disassembly was examined in situ by detection of the fluorescent product , resorufin , of ethoxyresorufin O-dealkylation .
	manualset3
147525	2	409653	5	NULL	NULL	0	NULL	cytochrome P450 CYP1A1/2 activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamics of cytochrome P450 CYP1A1/2 activity in the course of spheroid disassembly was examined in situ by detection of the fluorescent product , resorufin , of ethoxyresorufin O-dealkylation .
	manualset3
147526	3	409653	5	NULL	NULL	0	NULL	course 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamics of cytochrome P450 CYP1A1/2 activity in the course of spheroid disassembly was examined in situ by detection of the fluorescent product , resorufin , of ethoxyresorufin O-dealkylation .
	manualset3
147527	4	409653	5	NULL	NULL	0	NULL	spheroid disassembly	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamics of cytochrome P450 CYP1A1/2 activity in the course of spheroid disassembly was examined in situ by detection of the fluorescent product , resorufin , of ethoxyresorufin O-dealkylation .
	manualset3
147528	5	409653	5	NULL	NULL	0	NULL	detection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamics of cytochrome P450 CYP1A1/2 activity in the course of spheroid disassembly was examined in situ by detection of the fluorescent product , resorufin , of ethoxyresorufin O-dealkylation .
	manualset3
147529	6	409653	5	NULL	NULL	0	NULL	fluorescent product , resorufin	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamics of cytochrome P450 CYP1A1/2 activity in the course of spheroid disassembly was examined in situ by detection of the fluorescent product , resorufin , of ethoxyresorufin O-dealkylation .
	manualset3
147530	7	409653	5	NULL	NULL	0	NULL	ethoxyresorufin O-dealkylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamics of cytochrome P450 CYP1A1/2 activity in the course of spheroid disassembly was examined in situ by detection of the fluorescent product , resorufin , of ethoxyresorufin O-dealkylation .
	manualset3
147531	1	409654	5	NULL	NULL	0	NULL	dynamics 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamics of decay could be fitted well by Logistic model and Gompertz model , and no difference was observed between the fit goodness of the models .
	manualset3
147532	2	409654	5	NULL	NULL	0	NULL	decay 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamics of decay could be fitted well by Logistic model and Gompertz model , and no difference was observed between the fit goodness of the models .
	manualset3
147533	3	409654	5	NULL	NULL	0	NULL	Logistic model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamics of decay could be fitted well by Logistic model and Gompertz model , and no difference was observed between the fit goodness of the models .
	manualset3
147534	4	409654	5	NULL	NULL	0	NULL	Gompertz model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamics of decay could be fitted well by Logistic model and Gompertz model , and no difference was observed between the fit goodness of the models .
	manualset3
147535	5	409654	5	NULL	NULL	0	NULL	difference 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamics of decay could be fitted well by Logistic model and Gompertz model , and no difference was observed between the fit goodness of the models .
	manualset3
147536	6	409654	5	NULL	NULL	0	NULL	fit goodness 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamics of decay could be fitted well by Logistic model and Gompertz model , and no difference was observed between the fit goodness of the models .
	manualset3
147537	7	409654	5	NULL	NULL	0	NULL	models 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamics of decay could be fitted well by Logistic model and Gompertz model , and no difference was observed between the fit goodness of the models .
	manualset3
147538	1	409655	5	NULL	NULL	0	NULL	dynamics 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamics of met-enkephalin is considerably more complicated than that of the previously studied glycine oligomers ; met-enkephalin contains the interesting motions of phenyl groups and of side chains relative to the backbone , motions that are present in general flexible peptides .
	manualset3
147539	2	409655	5	NULL	NULL	NULL	NULL	Met-enkephalin	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The dynamics of met-enkephalin is considerably more complicated than that of the previously studied glycine oligomers ; met-enkephalin contains the interesting motions of phenyl groups and of side chains relative to the backbone , motions that are present in general flexible peptides .
	manualset3
147540	3	409655	5	NULL	NULL	0	NULL	glycine oligomers	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamics of met-enkephalin is considerably more complicated than that of the previously studied glycine oligomers ; met-enkephalin contains the interesting motions of phenyl groups and of side chains relative to the backbone , motions that are present in general flexible peptides .
	manualset3
147541	4	409655	5	NULL	NULL	0	NULL	met-enkephalin	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamics of met-enkephalin is considerably more complicated than that of the previously studied glycine oligomers ; met-enkephalin contains the interesting motions of phenyl groups and of side chains relative to the backbone , motions that are present in general flexible peptides .
	manualset3
147542	5	409655	5	NULL	NULL	0	NULL	motions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamics of met-enkephalin is considerably more complicated than that of the previously studied glycine oligomers ; met-enkephalin contains the interesting motions of phenyl groups and of side chains relative to the backbone , motions that are present in general flexible peptides .
	manualset3
147543	6	409655	5	NULL	NULL	0	NULL	phenyl groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamics of met-enkephalin is considerably more complicated than that of the previously studied glycine oligomers ; met-enkephalin contains the interesting motions of phenyl groups and of side chains relative to the backbone , motions that are present in general flexible peptides .
	manualset3
147544	7	409655	5	NULL	NULL	0	NULL	side chains	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamics of met-enkephalin is considerably more complicated than that of the previously studied glycine oligomers ; met-enkephalin contains the interesting motions of phenyl groups and of side chains relative to the backbone , motions that are present in general flexible peptides .
	manualset3
147545	8	409655	5	NULL	NULL	0	NULL	backbone , motions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamics of met-enkephalin is considerably more complicated than that of the previously studied glycine oligomers ; met-enkephalin contains the interesting motions of phenyl groups and of side chains relative to the backbone , motions that are present in general flexible peptides .
	manualset3
147546	9	409655	5	NULL	NULL	0	NULL	general flexible peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamics of met-enkephalin is considerably more complicated than that of the previously studied glycine oligomers ; met-enkephalin contains the interesting motions of phenyl groups and of side chains relative to the backbone , motions that are present in general flexible peptides .
	manualset3
147547	1	409656	5	NULL	NULL	0	NULL	dynamics 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamics of water , confined on a nanometer length scale ( 1.7 to 4.0 nm ) in sodium bis - ( 2-ethylhexyl ) sulfosuccinate reverse micelles , is directly investigated using frequency resolved infrared vibrational echo experiments .
	manualset3
147548	2	409656	5	NULL	NULL	0	NULL	water 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamics of water , confined on a nanometer length scale ( 1.7 to 4.0 nm ) in sodium bis - ( 2-ethylhexyl ) sulfosuccinate reverse micelles , is directly investigated using frequency resolved infrared vibrational echo experiments .
	manualset3
147549	3	409656	5	NULL	NULL	0	NULL	nanometer length scale	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamics of water , confined on a nanometer length scale ( 1.7 to 4.0 nm ) in sodium bis - ( 2-ethylhexyl ) sulfosuccinate reverse micelles , is directly investigated using frequency resolved infrared vibrational echo experiments .
	manualset3
147550	4	409656	5	NULL	NULL	0	NULL	1.7 to 4.0 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamics of water , confined on a nanometer length scale ( 1.7 to 4.0 nm ) in sodium bis - ( 2-ethylhexyl ) sulfosuccinate reverse micelles , is directly investigated using frequency resolved infrared vibrational echo experiments .
	manualset3
147551	5	409656	5	NULL	NULL	0	NULL	sodium bis - ( 2-ethylhexyl ) sulfosuccinate reverse micelles	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamics of water , confined on a nanometer length scale ( 1.7 to 4.0 nm ) in sodium bis - ( 2-ethylhexyl ) sulfosuccinate reverse micelles , is directly investigated using frequency resolved infrared vibrational echo experiments .
	manualset3
147552	6	409656	5	NULL	NULL	0	NULL	frequency resolved infrared vibrational echo experiments 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The dynamics of water , confined on a nanometer length scale ( 1.7 to 4.0 nm ) in sodium bis - ( 2-ethylhexyl ) sulfosuccinate reverse micelles , is directly investigated using frequency resolved infrared vibrational echo experiments .
	manualset3
147553	1	409657	5	NULL	NULL	0	NULL	dystrophic muscle simulator 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The dystrophic muscle simulator is freely accessible via the Genethon web site ( www.genethon.fr ) , and in the online version via http : @ www.wiley.co.uk / genmed .
	manualset3
147554	2	409657	5	NULL	NULL	0	NULL	Genethon web site ( www.genethon.fr ) 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The dystrophic muscle simulator is freely accessible via the Genethon web site ( www.genethon.fr ) , and in the online version via http : @ www.wiley.co.uk / genmed .
	manualset3
147555	3	409657	5	NULL	NULL	0	NULL	online version	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The dystrophic muscle simulator is freely accessible via the Genethon web site ( www.genethon.fr ) , and in the online version via http : @ www.wiley.co.uk / genmed .
	manualset3
147556	4	409657	5	NULL	NULL	0	NULL	http : @ www.wiley.co.uk / genmed	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The dystrophic muscle simulator is freely accessible via the Genethon web site ( www.genethon.fr ) , and in the online version via http : @ www.wiley.co.uk / genmed .
	manualset3
147557	1	409658	5	NULL	NULL	0	NULL	 early peak	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The early peak to PNS at 4 or 8 Hz was abolished by prazosin , an alpha1-adrenoceptor antagonist , while the late one still remained , although it was markedly inhibited .
	manualset3
147558	2	409658	5	NULL	NULL	0	NULL	PNS 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The early peak to PNS at 4 or 8 Hz was abolished by prazosin , an alpha1-adrenoceptor antagonist , while the late one still remained , although it was markedly inhibited .
	manualset3
147559	3	409658	5	NULL	NULL	0	NULL	4 or 8 Hz	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The early peak to PNS at 4 or 8 Hz was abolished by prazosin , an alpha1-adrenoceptor antagonist , while the late one still remained , although it was markedly inhibited .
	manualset3
147560	4	409658	5	NULL	NULL	NULL	NULL	prazosin , an alpha1-adrenoceptor antagonist	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The early peak to PNS at 4 or 8 Hz was abolished by prazosin , an alpha1-adrenoceptor antagonist , while the late one still remained , although it was markedly inhibited .
	manualset3
147561	1	409659	5	NULL	NULL	0	NULL	ease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ease or difficulty of picture recognition is shown to vary with complexity , familiarity , and categorical information .
	manualset3
147562	2	409659	5	NULL	NULL	0	NULL	difficulty 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ease or difficulty of picture recognition is shown to vary with complexity , familiarity , and categorical information .
	manualset3
147563	3	409659	5	NULL	NULL	0	NULL	picture recognition 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ease or difficulty of picture recognition is shown to vary with complexity , familiarity , and categorical information .
	manualset3
147564	4	409659	5	NULL	NULL	0	NULL	complexity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ease or difficulty of picture recognition is shown to vary with complexity , familiarity , and categorical information .
	manualset3
147565	5	409659	5	NULL	NULL	0	NULL	familiarity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ease or difficulty of picture recognition is shown to vary with complexity , familiarity , and categorical information .
	manualset3
147566	6	409659	5	NULL	NULL	0	NULL	categorical information	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ease or difficulty of picture recognition is shown to vary with complexity , familiarity , and categorical information .
	manualset3
147567	1	409660	5	NULL	NULL	0	NULL	eating disorders medicine cabinet	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The eating disorders medicine cabinet revisited : a clinician 's guide to ipecac and laxatives .
	manualset3
147568	2	409660	5	NULL	NULL	0	NULL	clinician 's guide	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The eating disorders medicine cabinet revisited : a clinician 's guide to ipecac and laxatives .
	manualset3
147569	3	409660	5	NULL	NULL	0	NULL	ipecac	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The eating disorders medicine cabinet revisited : a clinician 's guide to ipecac and laxatives .
	manualset3
147570	4	409660	5	NULL	NULL	0	NULL	laxatives	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The eating disorders medicine cabinet revisited : a clinician 's guide to ipecac and laxatives .
	manualset3
147571	1	409661	5	NULL	NULL	0	NULL	eccentric exercise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The eccentric exercise caused lengthening of kinematic parameters including total movement time and time to peak velocity .
	manualset3
147572	2	409661	5	NULL	NULL	0	NULL	kinematic parameters	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The eccentric exercise caused lengthening of kinematic parameters including total movement time and time to peak velocity .
	manualset3
147573	3	409661	5	NULL	NULL	0	NULL	total movement time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The eccentric exercise caused lengthening of kinematic parameters including total movement time and time to peak velocity .
	manualset3
147574	4	409661	5	NULL	NULL	0	NULL	time to peak velocity	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The eccentric exercise caused lengthening of kinematic parameters including total movement time and time to peak velocity .
	manualset3
147575	1	409662	5	NULL	NULL	0	NULL	humankind 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The ecologically most significant respect in which humankind now dominates all other terrestrial species is in its scientific understanding and technological manipulation of the world .
	manualset3
147576	2	409662	5	NULL	NULL	0	NULL	terrestrial species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The ecologically most significant respect in which humankind now dominates all other terrestrial species is in its scientific understanding and technological manipulation of the world .
	manualset3
147577	3	409662	5	NULL	NULL	0	NULL	scientific understanding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ecologically most significant respect in which humankind now dominates all other terrestrial species is in its scientific understanding and technological manipulation of the world .
	manualset3
147578	4	409662	5	NULL	NULL	0	NULL	technological manipulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ecologically most significant respect in which humankind now dominates all other terrestrial species is in its scientific understanding and technological manipulation of the world .
	manualset3
147579	5	409662	5	NULL	NULL	0	NULL	world 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The ecologically most significant respect in which humankind now dominates all other terrestrial species is in its scientific understanding and technological manipulation of the world .
	manualset3
147580	1	409663	5	NULL	NULL	0	NULL	ecology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ecology of the pathogen is discussed with emphasis on host range , dispersal and primary source of infection .
	manualset3
147581	2	409663	5	NULL	NULL	0	NULL	pathogen 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The ecology of the pathogen is discussed with emphasis on host range , dispersal and primary source of infection .
	manualset3
147582	3	409663	5	NULL	NULL	0	NULL	emphasis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ecology of the pathogen is discussed with emphasis on host range , dispersal and primary source of infection .
	manualset3
147583	4	409663	5	NULL	NULL	0	NULL	host range 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The ecology of the pathogen is discussed with emphasis on host range , dispersal and primary source of infection .
	manualset3
147584	5	409663	5	NULL	NULL	0	NULL	source of infection	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ecology of the pathogen is discussed with emphasis on host range , dispersal and primary source of infection .
	manualset3
147585	1	409664	5	NULL	NULL	0	NULL	economic margin	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The economic margin , calculated as income achieved minus costs , was greatest for LUC , intermediate for LUC + Feedlot and lowest for Feedlot treatment .
	manualset3
147586	2	409664	5	NULL	NULL	0	NULL	income 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The economic margin , calculated as income achieved minus costs , was greatest for LUC , intermediate for LUC + Feedlot and lowest for Feedlot treatment .
	manualset3
147587	3	409664	5	NULL	NULL	0	NULL	costs 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The economic margin , calculated as income achieved minus costs , was greatest for LUC , intermediate for LUC + Feedlot and lowest for Feedlot treatment .
	manualset3
147588	4	409664	5	NULL	NULL	0	NULL	LUC 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The economic margin , calculated as income achieved minus costs , was greatest for LUC , intermediate for LUC + Feedlot and lowest for Feedlot treatment .
	manualset3
147589	5	409664	5	NULL	NULL	0	NULL	LUC + Feedlot	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The economic margin , calculated as income achieved minus costs , was greatest for LUC , intermediate for LUC + Feedlot and lowest for Feedlot treatment .
	manualset3
147590	6	409664	5	NULL	NULL	0	NULL	Feedlot treatment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The economic margin , calculated as income achieved minus costs , was greatest for LUC , intermediate for LUC + Feedlot and lowest for Feedlot treatment .
	manualset3
147591	1	409665	5	NULL	NULL	0	NULL	ectonucleotidase cd39/ENTPDase1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The ectonucleotidase cd39/ENTPDase1 modulates purinergic-mediated microglial migration .
	manualset3
147592	2	409665	5	NULL	NULL	0	NULL	purinergic-mediated microglial migration 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ectonucleotidase cd39/ENTPDase1 modulates purinergic-mediated microglial migration .
	manualset3
147593	1	409666	5	NULL	NULL	0	NULL	specific adenosine triphosphatase ( ATPase ) staining technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A specific adenosine triphosphatase ( ATPase ) staining technique was used to identify epidermal LC .
	manualset3
147594	2	409666	5	NULL	NULL	0	NULL	epidermal LC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A specific adenosine triphosphatase ( ATPase ) staining technique was used to identify epidermal LC .
	manualset3
147595	1	409667	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect correlates with the production of an ATP-dependent ds DNA exonuclease in recB/R1drd -19 cells .
	manualset3
147596	2	409667	5	NULL	NULL	0	NULL	production 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect correlates with the production of an ATP-dependent ds DNA exonuclease in recB/R1drd -19 cells .
	manualset3
147597	3	409667	5	NULL	NULL	0	NULL	ATP-dependent ds DNA exonuclease	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect correlates with the production of an ATP-dependent ds DNA exonuclease in recB/R1drd -19 cells .
	manualset3
147598	4	409667	5	NULL	NULL	0	NULL	recB/R1drd -19 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect correlates with the production of an ATP-dependent ds DNA exonuclease in recB/R1drd -19 cells .
	manualset3
147599	1	409668	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect found on MRI was not reflected in a corresponding change in the QoL .
	manualset3
147600	2	409668	5	NULL	NULL	0	NULL	MRI 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect found on MRI was not reflected in a corresponding change in the QoL .
	manualset3
147601	3	409668	5	NULL	NULL	0	NULL	corresponding change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect found on MRI was not reflected in a corresponding change in the QoL .
	manualset3
147602	4	409668	5	NULL	NULL	0	NULL	QoL 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect found on MRI was not reflected in a corresponding change in the QoL .
	manualset3
147603	1	409669	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of a beta adrenergic blocking agent on chemical changes in isoproterenol-induced myocardial necrosis .
	manualset3
147604	2	409669	5	NULL	NULL	0	NULL	beta adrenergic blocking agent	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of a beta adrenergic blocking agent on chemical changes in isoproterenol-induced myocardial necrosis .
	manualset3
147605	3	409669	5	NULL	NULL	0	NULL	chemical changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of a beta adrenergic blocking agent on chemical changes in isoproterenol-induced myocardial necrosis .
	manualset3
147606	4	409669	5	NULL	NULL	0	NULL	isoproterenol-induced myocardial necrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of a beta adrenergic blocking agent on chemical changes in isoproterenol-induced myocardial necrosis .
	manualset3
147607	1	409670	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of a moderate heat stress on cardiovascular responses was studied : group I consisted of 15 healthy non-pregnant women , group II of 23 women 13-14 weeks pregnant and group III of 23 women 36-37 weeks pregnant .
	manualset3
147608	2	409670	5	NULL	NULL	0	NULL	moderate heat stress 	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of a moderate heat stress on cardiovascular responses was studied : group I consisted of 15 healthy non-pregnant women , group II of 23 women 13-14 weeks pregnant and group III of 23 women 36-37 weeks pregnant .
	manualset3
147609	3	409670	5	NULL	NULL	0	NULL	cardiovascular responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of a moderate heat stress on cardiovascular responses was studied : group I consisted of 15 healthy non-pregnant women , group II of 23 women 13-14 weeks pregnant and group III of 23 women 36-37 weeks pregnant .
	manualset3
147610	4	409670	5	NULL	NULL	0	NULL	group I 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of a moderate heat stress on cardiovascular responses was studied : group I consisted of 15 healthy non-pregnant women , group II of 23 women 13-14 weeks pregnant and group III of 23 women 36-37 weeks pregnant .
	manualset3
147611	5	409670	5	NULL	NULL	0	NULL	15 healthy non-pregnant women 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of a moderate heat stress on cardiovascular responses was studied : group I consisted of 15 healthy non-pregnant women , group II of 23 women 13-14 weeks pregnant and group III of 23 women 36-37 weeks pregnant .
	manualset3
147612	6	409670	5	NULL	NULL	0	NULL	group II	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of a moderate heat stress on cardiovascular responses was studied : group I consisted of 15 healthy non-pregnant women , group II of 23 women 13-14 weeks pregnant and group III of 23 women 36-37 weeks pregnant .
	manualset3
147613	7	409670	5	NULL	NULL	0	NULL	23 women 13-14 weeks pregnant	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of a moderate heat stress on cardiovascular responses was studied : group I consisted of 15 healthy non-pregnant women , group II of 23 women 13-14 weeks pregnant and group III of 23 women 36-37 weeks pregnant .
	manualset3
147614	8	409670	5	NULL	NULL	0	NULL	group III 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of a moderate heat stress on cardiovascular responses was studied : group I consisted of 15 healthy non-pregnant women , group II of 23 women 13-14 weeks pregnant and group III of 23 women 36-37 weeks pregnant .
	manualset3
147615	9	409670	5	NULL	NULL	0	NULL	23 women 36-37 weeks pregnant 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of a moderate heat stress on cardiovascular responses was studied : group I consisted of 15 healthy non-pregnant women , group II of 23 women 13-14 weeks pregnant and group III of 23 women 36-37 weeks pregnant .
	manualset3
147616	1	409671	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of a passive change from supine to 25-degree head-up tilted position on left ventricular volume was studied by echocardiography and other noninvasive techniques in 18 normal subjects , 6 patients with compensated LV volume overloading , and 12 patients with LV failure .
	manualset3
147617	2	409671	5	NULL	NULL	0	NULL	passive change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of a passive change from supine to 25-degree head-up tilted position on left ventricular volume was studied by echocardiography and other noninvasive techniques in 18 normal subjects , 6 patients with compensated LV volume overloading , and 12 patients with LV failure .
	manualset3
147618	3	409671	5	NULL	NULL	0	NULL	supine 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of a passive change from supine to 25-degree head-up tilted position on left ventricular volume was studied by echocardiography and other noninvasive techniques in 18 normal subjects , 6 patients with compensated LV volume overloading , and 12 patients with LV failure .
	manualset3
147619	4	409671	5	NULL	NULL	0	NULL	25-degree head-up tilted position	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of a passive change from supine to 25-degree head-up tilted position on left ventricular volume was studied by echocardiography and other noninvasive techniques in 18 normal subjects , 6 patients with compensated LV volume overloading , and 12 patients with LV failure .
	manualset3
147620	5	409671	5	NULL	NULL	0	NULL	left ventricular volume 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of a passive change from supine to 25-degree head-up tilted position on left ventricular volume was studied by echocardiography and other noninvasive techniques in 18 normal subjects , 6 patients with compensated LV volume overloading , and 12 patients with LV failure .
	manualset3
147621	6	409671	5	NULL	NULL	0	NULL	echocardiography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of a passive change from supine to 25-degree head-up tilted position on left ventricular volume was studied by echocardiography and other noninvasive techniques in 18 normal subjects , 6 patients with compensated LV volume overloading , and 12 patients with LV failure .
	manualset3
147622	7	409671	5	NULL	NULL	0	NULL	noninvasive techniques	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of a passive change from supine to 25-degree head-up tilted position on left ventricular volume was studied by echocardiography and other noninvasive techniques in 18 normal subjects , 6 patients with compensated LV volume overloading , and 12 patients with LV failure .
	manualset3
147623	8	409671	5	NULL	NULL	0	NULL	18 normal subjects	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of a passive change from supine to 25-degree head-up tilted position on left ventricular volume was studied by echocardiography and other noninvasive techniques in 18 normal subjects , 6 patients with compensated LV volume overloading , and 12 patients with LV failure .
	manualset3
147624	9	409671	5	NULL	NULL	0	NULL	6 patients 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of a passive change from supine to 25-degree head-up tilted position on left ventricular volume was studied by echocardiography and other noninvasive techniques in 18 normal subjects , 6 patients with compensated LV volume overloading , and 12 patients with LV failure .
	manualset3
147625	10	409671	5	NULL	NULL	0	NULL	compensated LV volume overloading	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of a passive change from supine to 25-degree head-up tilted position on left ventricular volume was studied by echocardiography and other noninvasive techniques in 18 normal subjects , 6 patients with compensated LV volume overloading , and 12 patients with LV failure .
	manualset3
147626	11	409671	5	NULL	NULL	0	NULL	12 patients	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of a passive change from supine to 25-degree head-up tilted position on left ventricular volume was studied by echocardiography and other noninvasive techniques in 18 normal subjects , 6 patients with compensated LV volume overloading , and 12 patients with LV failure .
	manualset3
147627	12	409671	5	NULL	NULL	0	NULL	LV failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of a passive change from supine to 25-degree head-up tilted position on left ventricular volume was studied by echocardiography and other noninvasive techniques in 18 normal subjects , 6 patients with compensated LV volume overloading , and 12 patients with LV failure .
	manualset3
147628	1	409672	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of acetylator status was seen as higher C ( max ) and AUC of OR-1855 in slow acetylators .
	manualset3
147629	2	409672	5	NULL	NULL	0	NULL	acetylator status 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of acetylator status was seen as higher C ( max ) and AUC of OR-1855 in slow acetylators .
	manualset3
147630	3	409672	5	NULL	NULL	0	NULL	higher C ( max ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of acetylator status was seen as higher C ( max ) and AUC of OR-1855 in slow acetylators .
	manualset3
147631	4	409672	5	NULL	NULL	0	NULL	AUC of OR-1855	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of acetylator status was seen as higher C ( max ) and AUC of OR-1855 in slow acetylators .
	manualset3
147632	5	409672	5	NULL	NULL	0	NULL	slow acetylators	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of acetylator status was seen as higher C ( max ) and AUC of OR-1855 in slow acetylators .
	manualset3
147633	1	409673	5	NULL	NULL	0	NULL	specific adenylate cyclase inhibitor , cis-N - ( 2-phenylcyclopentyl ) - azacyclotridec-1-en-2-amine ( MDL-12 , 330 A ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A specific adenylate cyclase inhibitor , cis-N - ( 2-phenylcyclopentyl ) - azacyclotridec-1-en-2-amine ( MDL-12 , 330 A ) promoted the growth of the yeast form .
	manualset3
147634	2	409673	5	NULL	NULL	0	NULL	growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A specific adenylate cyclase inhibitor , cis-N - ( 2-phenylcyclopentyl ) - azacyclotridec-1-en-2-amine ( MDL-12 , 330 A ) promoted the growth of the yeast form .
	manualset3
147635	3	409673	5	NULL	NULL	0	NULL	yeast form	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A specific adenylate cyclase inhibitor , cis-N - ( 2-phenylcyclopentyl ) - azacyclotridec-1-en-2-amine ( MDL-12 , 330 A ) promoted the growth of the yeast form .
	manualset3
147636	1	409674	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of acute cold exposure on the concentration of glucagon in the blood was investigated in man and in intact and adrenalectomized rats .
	manualset3
147637	2	409674	5	NULL	NULL	0	NULL	acute cold exposure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of acute cold exposure on the concentration of glucagon in the blood was investigated in man and in intact and adrenalectomized rats .
	manualset3
147638	3	409674	5	NULL	NULL	0	NULL	concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of acute cold exposure on the concentration of glucagon in the blood was investigated in man and in intact and adrenalectomized rats .
	manualset3
147639	4	409674	5	NULL	NULL	0	NULL	glucagon 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of acute cold exposure on the concentration of glucagon in the blood was investigated in man and in intact and adrenalectomized rats .
	manualset3
147640	5	409674	5	NULL	NULL	0	NULL	blood 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of acute cold exposure on the concentration of glucagon in the blood was investigated in man and in intact and adrenalectomized rats .
	manualset3
147641	6	409674	5	NULL	NULL	0	NULL	man 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of acute cold exposure on the concentration of glucagon in the blood was investigated in man and in intact and adrenalectomized rats .
	manualset3
147642	7	409674	5	NULL	NULL	0	NULL	intact rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of acute cold exposure on the concentration of glucagon in the blood was investigated in man and in intact and adrenalectomized rats .
	manualset3
147643	8	409674	5	NULL	NULL	0	NULL	adrenalectomized rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of acute cold exposure on the concentration of glucagon in the blood was investigated in man and in intact and adrenalectomized rats .
	manualset3
147644	1	409675	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of adenosine receptor blockade and adrenergic blockade on myocardial stunning ( left anterior descending coronary artery ( LAD ) occluded for 10 min and reperfused for 180 min ) was studied in 38 open-chest cats .
	manualset3
147645	2	409675	5	NULL	NULL	0	NULL	adenosine receptor blockade 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of adenosine receptor blockade and adrenergic blockade on myocardial stunning ( left anterior descending coronary artery ( LAD ) occluded for 10 min and reperfused for 180 min ) was studied in 38 open-chest cats .
	manualset3
147646	3	409675	5	NULL	NULL	0	NULL	adrenergic blockade	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of adenosine receptor blockade and adrenergic blockade on myocardial stunning ( left anterior descending coronary artery ( LAD ) occluded for 10 min and reperfused for 180 min ) was studied in 38 open-chest cats .
	manualset3
147647	4	409675	5	NULL	NULL	0	NULL	myocardial stunning	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of adenosine receptor blockade and adrenergic blockade on myocardial stunning ( left anterior descending coronary artery ( LAD ) occluded for 10 min and reperfused for 180 min ) was studied in 38 open-chest cats .
	manualset3
147648	5	409675	5	NULL	NULL	0	NULL	left anterior descending coronary artery ( LAD ) 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of adenosine receptor blockade and adrenergic blockade on myocardial stunning ( left anterior descending coronary artery ( LAD ) occluded for 10 min and reperfused for 180 min ) was studied in 38 open-chest cats .
	manualset3
147649	6	409675	5	NULL	NULL	0	NULL	10 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of adenosine receptor blockade and adrenergic blockade on myocardial stunning ( left anterior descending coronary artery ( LAD ) occluded for 10 min and reperfused for 180 min ) was studied in 38 open-chest cats .
	manualset3
147650	7	409675	5	NULL	NULL	0	NULL	180 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of adenosine receptor blockade and adrenergic blockade on myocardial stunning ( left anterior descending coronary artery ( LAD ) occluded for 10 min and reperfused for 180 min ) was studied in 38 open-chest cats .
	manualset3
147651	8	409675	5	NULL	NULL	0	NULL	38 open-chest cats	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of adenosine receptor blockade and adrenergic blockade on myocardial stunning ( left anterior descending coronary artery ( LAD ) occluded for 10 min and reperfused for 180 min ) was studied in 38 open-chest cats .
	manualset3
147652	1	409676	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of alertness and visual attention on optokinetic nystagmus ( OKN ) and optokinetic after-nystagmus ( OKAN ) was studied in 20 volunteers .
	manualset3
147653	2	409676	5	NULL	NULL	0	NULL	alertness 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of alertness and visual attention on optokinetic nystagmus ( OKN ) and optokinetic after-nystagmus ( OKAN ) was studied in 20 volunteers .
	manualset3
147654	3	409676	5	NULL	NULL	0	NULL	visual attention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of alertness and visual attention on optokinetic nystagmus ( OKN ) and optokinetic after-nystagmus ( OKAN ) was studied in 20 volunteers .
	manualset3
147655	4	409676	5	NULL	NULL	0	NULL	optokinetic nystagmus ( OKN ) 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of alertness and visual attention on optokinetic nystagmus ( OKN ) and optokinetic after-nystagmus ( OKAN ) was studied in 20 volunteers .
	manualset3
147656	5	409676	5	NULL	NULL	0	NULL	optokinetic after-nystagmus ( OKAN )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of alertness and visual attention on optokinetic nystagmus ( OKN ) and optokinetic after-nystagmus ( OKAN ) was studied in 20 volunteers .
	manualset3
147657	6	409676	5	NULL	NULL	0	NULL	20 volunteers	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of alertness and visual attention on optokinetic nystagmus ( OKN ) and optokinetic after-nystagmus ( OKAN ) was studied in 20 volunteers .
	manualset3
147658	1	409677	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of aluminum incorporation on silver metal quantum dots formation in the alumino-silicate glass film processed by sol-gel process was investigated .
	manualset3
147659	2	409677	5	NULL	NULL	0	NULL	aluminum incorporation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of aluminum incorporation on silver metal quantum dots formation in the alumino-silicate glass film processed by sol-gel process was investigated .
	manualset3
147660	3	409677	5	NULL	NULL	0	NULL	silver metal quantum dots formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of aluminum incorporation on silver metal quantum dots formation in the alumino-silicate glass film processed by sol-gel process was investigated .
	manualset3
147661	4	409677	5	NULL	NULL	0	NULL	alumino-silicate glass film	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of aluminum incorporation on silver metal quantum dots formation in the alumino-silicate glass film processed by sol-gel process was investigated .
	manualset3
147662	5	409677	5	NULL	NULL	0	NULL	sol-gel process	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of aluminum incorporation on silver metal quantum dots formation in the alumino-silicate glass film processed by sol-gel process was investigated .
	manualset3
147663	1	409678	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of androgens on P1 expression was also investigated .
	manualset3
147664	2	409678	5	NULL	NULL	0	NULL	androgens	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of androgens on P1 expression was also investigated .
	manualset3
147665	3	409678	5	NULL	NULL	0	NULL	P1 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of androgens on P1 expression was also investigated .
	manualset3
147666	1	409679	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of atropine , ergotamine , and pituitrin on phlorhizin glycosuria .
	manualset3
147667	2	409679	5	NULL	NULL	0	NULL	atropine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of atropine , ergotamine , and pituitrin on phlorhizin glycosuria .
	manualset3
147668	3	409679	5	NULL	NULL	0	NULL	ergotamine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of atropine , ergotamine , and pituitrin on phlorhizin glycosuria .
	manualset3
147669	4	409679	5	NULL	NULL	0	NULL	pituitrin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of atropine , ergotamine , and pituitrin on phlorhizin glycosuria .
	manualset3
147670	5	409679	5	NULL	NULL	0	NULL	phlorhizin glycosuria	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of atropine , ergotamine , and pituitrin on phlorhizin glycosuria .
	manualset3
147671	1	409680	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of calcium antagonists on histamine and leukotriene-induced tracheal microvascular permeability in the guinea pig .
	manualset3
147672	2	409680	5	NULL	NULL	0	NULL	calcium antagonists	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of calcium antagonists on histamine and leukotriene-induced tracheal microvascular permeability in the guinea pig .
	manualset3
147673	3	409680	5	NULL	NULL	0	NULL	histamine-induced tracheal microvascular permeability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of calcium antagonists on histamine and leukotriene-induced tracheal microvascular permeability in the guinea pig .
	manualset3
147674	4	409680	5	NULL	NULL	0	NULL	leukotriene-induced tracheal microvascular permeability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of calcium antagonists on histamine and leukotriene-induced tracheal microvascular permeability in the guinea pig .
	manualset3
147675	5	409680	5	NULL	NULL	0	NULL	guinea pig	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of calcium antagonists on histamine and leukotriene-induced tracheal microvascular permeability in the guinea pig .
	manualset3
147676	1	409681	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of cetylpyridinium chloride ( CPC ) , a cationic detergent , on the biosynthetic ability of the well known synthesizor of nucleotides Brevibacterium ammoniagenes ATCC 6872 was studied .
	manualset3
147677	2	409681	5	NULL	NULL	0	NULL	cetylpyridinium chloride ( CPC ) , a cationic detergent	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of cetylpyridinium chloride ( CPC ) , a cationic detergent , on the biosynthetic ability of the well known synthesizor of nucleotides Brevibacterium ammoniagenes ATCC 6872 was studied .
	manualset3
147678	3	409681	5	NULL	NULL	0	NULL	biosynthetic ability 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of cetylpyridinium chloride ( CPC ) , a cationic detergent , on the biosynthetic ability of the well known synthesizor of nucleotides Brevibacterium ammoniagenes ATCC 6872 was studied .
	manualset3
147679	4	409681	5	NULL	NULL	0	NULL	synthesizor of nucleotides Brevibacterium ammoniagenes ATCC 6872	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of cetylpyridinium chloride ( CPC ) , a cationic detergent , on the biosynthetic ability of the well known synthesizor of nucleotides Brevibacterium ammoniagenes ATCC 6872 was studied .
	manualset3
147680	1	409682	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of chlordiazepoxide and fluphenazine on critical flicker frequency .
	manualset3
147681	2	409682	5	NULL	NULL	0	NULL	chlordiazepoxide 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of chlordiazepoxide and fluphenazine on critical flicker frequency .
	manualset3
147682	3	409682	5	NULL	NULL	0	NULL	fluphenazine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of chlordiazepoxide and fluphenazine on critical flicker frequency .
	manualset3
147683	4	409682	5	NULL	NULL	0	NULL	critical flicker frequency 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of chlordiazepoxide and fluphenazine on critical flicker frequency .
	manualset3
147684	1	409683	5	NULL	NULL	0	NULL	specific enzymeimmunoassay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A specific enzymeimmunoassay for progesterone in human plasma .
	manualset3
147685	2	409683	5	NULL	NULL	0	NULL	progesterone 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A specific enzymeimmunoassay for progesterone in human plasma .
	manualset3
147686	3	409683	5	NULL	NULL	0	NULL	human plasma	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A specific enzymeimmunoassay for progesterone in human plasma .
	manualset3
147687	1	409684	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of chronic , severe diabetes mellitus on the morphology , blood flow regulation , and tissue PO2 of the cerebral cortex was evaluated in adult rats .
	manualset3
147688	2	409684	5	NULL	NULL	0	NULL	diabetes mellitus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of chronic , severe diabetes mellitus on the morphology , blood flow regulation , and tissue PO2 of the cerebral cortex was evaluated in adult rats .
	manualset3
147689	3	409684	5	NULL	NULL	0	NULL	morphology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of chronic , severe diabetes mellitus on the morphology , blood flow regulation , and tissue PO2 of the cerebral cortex was evaluated in adult rats .
	manualset3
147690	4	409684	5	NULL	NULL	0	NULL	blood flow regulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of chronic , severe diabetes mellitus on the morphology , blood flow regulation , and tissue PO2 of the cerebral cortex was evaluated in adult rats .
	manualset3
147691	5	409684	5	NULL	NULL	0	NULL	tissue PO2 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of chronic , severe diabetes mellitus on the morphology , blood flow regulation , and tissue PO2 of the cerebral cortex was evaluated in adult rats .
	manualset3
147692	6	409684	5	NULL	NULL	0	NULL	cerebral cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of chronic , severe diabetes mellitus on the morphology , blood flow regulation , and tissue PO2 of the cerebral cortex was evaluated in adult rats .
	manualset3
147693	7	409684	5	NULL	NULL	0	NULL	adult rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of chronic , severe diabetes mellitus on the morphology , blood flow regulation , and tissue PO2 of the cerebral cortex was evaluated in adult rats .
	manualset3
147694	1	409685	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of clomipramine ( CMI ) , a tricyclic antidepressant , was studied on an acute inflammatory pain model in an attempt to understand its potential antinociceptive activity , the involvement of a central and/or peripheral component and its influence on the inflammatory process .
	manualset3
147695	2	409685	5	NULL	NULL	0	NULL	clomipramine ( CMI ) , a tricyclic antidepressant	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of clomipramine ( CMI ) , a tricyclic antidepressant , was studied on an acute inflammatory pain model in an attempt to understand its potential antinociceptive activity , the involvement of a central and/or peripheral component and its influence on the inflammatory process .
	manualset3
147696	3	409685	5	NULL	NULL	0	NULL	acute inflammatory pain model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of clomipramine ( CMI ) , a tricyclic antidepressant , was studied on an acute inflammatory pain model in an attempt to understand its potential antinociceptive activity , the involvement of a central and/or peripheral component and its influence on the inflammatory process .
	manualset3
147697	4	409685	5	NULL	NULL	0	NULL	potential antinociceptive activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of clomipramine ( CMI ) , a tricyclic antidepressant , was studied on an acute inflammatory pain model in an attempt to understand its potential antinociceptive activity , the involvement of a central and/or peripheral component and its influence on the inflammatory process .
	manualset3
147698	5	409685	5	NULL	NULL	0	NULL	involvement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of clomipramine ( CMI ) , a tricyclic antidepressant , was studied on an acute inflammatory pain model in an attempt to understand its potential antinociceptive activity , the involvement of a central and/or peripheral component and its influence on the inflammatory process .
	manualset3
147699	6	409685	5	NULL	NULL	0	NULL	central and/or peripheral component	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of clomipramine ( CMI ) , a tricyclic antidepressant , was studied on an acute inflammatory pain model in an attempt to understand its potential antinociceptive activity , the involvement of a central and/or peripheral component and its influence on the inflammatory process .
	manualset3
147700	7	409685	5	NULL	NULL	0	NULL	influence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of clomipramine ( CMI ) , a tricyclic antidepressant , was studied on an acute inflammatory pain model in an attempt to understand its potential antinociceptive activity , the involvement of a central and/or peripheral component and its influence on the inflammatory process .
	manualset3
147701	8	409685	5	NULL	NULL	0	NULL	inflammatory process	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of clomipramine ( CMI ) , a tricyclic antidepressant , was studied on an acute inflammatory pain model in an attempt to understand its potential antinociceptive activity , the involvement of a central and/or peripheral component and its influence on the inflammatory process .
	manualset3
147702	1	409686	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of conjoining therapy to diagnosis will bring about a more ethical balance between the immediate risks and benefits of prenatal diagnosis .
	manualset3
147703	2	409686	5	NULL	NULL	0	NULL	conjoining therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of conjoining therapy to diagnosis will bring about a more ethical balance between the immediate risks and benefits of prenatal diagnosis .
	manualset3
147704	3	409686	5	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of conjoining therapy to diagnosis will bring about a more ethical balance between the immediate risks and benefits of prenatal diagnosis .
	manualset3
147705	4	409686	5	NULL	NULL	0	NULL	ethical balance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of conjoining therapy to diagnosis will bring about a more ethical balance between the immediate risks and benefits of prenatal diagnosis .
	manualset3
147706	5	409686	5	NULL	NULL	0	NULL	immediate risks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of conjoining therapy to diagnosis will bring about a more ethical balance between the immediate risks and benefits of prenatal diagnosis .
	manualset3
147707	6	409686	5	NULL	NULL	0	NULL	benefits 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of conjoining therapy to diagnosis will bring about a more ethical balance between the immediate risks and benefits of prenatal diagnosis .
	manualset3
147708	7	409686	5	NULL	NULL	0	NULL	prenatal diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of conjoining therapy to diagnosis will bring about a more ethical balance between the immediate risks and benefits of prenatal diagnosis .
	manualset3
147709	1	409687	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of culturing 2 and 5 ml of blood in 18 ml of supplemented peptone broth I ( SPB I ) and 45 ml of supplemented broth II ( SPB II ) respectively , was compared .
	manualset3
147710	2	409687	5	NULL	NULL	NULL	NULL	2 ml	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The effect of culturing 2 and 5 ml of blood in 18 ml of supplemented peptone broth I ( SPB I ) and 45 ml of supplemented broth II ( SPB II ) respectively , was compared .
	manualset3
147711	3	409687	5	NULL	NULL	0	NULL	5 ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of culturing 2 and 5 ml of blood in 18 ml of supplemented peptone broth I ( SPB I ) and 45 ml of supplemented broth II ( SPB II ) respectively , was compared .
	manualset3
147712	4	409687	5	NULL	NULL	0	NULL	blood 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of culturing 2 and 5 ml of blood in 18 ml of supplemented peptone broth I ( SPB I ) and 45 ml of supplemented broth II ( SPB II ) respectively , was compared .
	manualset3
147713	5	409687	5	NULL	NULL	0	NULL	18 ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of culturing 2 and 5 ml of blood in 18 ml of supplemented peptone broth I ( SPB I ) and 45 ml of supplemented broth II ( SPB II ) respectively , was compared .
	manualset3
147714	6	409687	5	NULL	NULL	0	NULL	supplemented peptone broth I ( SPB I )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of culturing 2 and 5 ml of blood in 18 ml of supplemented peptone broth I ( SPB I ) and 45 ml of supplemented broth II ( SPB II ) respectively , was compared .
	manualset3
147715	7	409687	5	NULL	NULL	0	NULL	45 ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of culturing 2 and 5 ml of blood in 18 ml of supplemented peptone broth I ( SPB I ) and 45 ml of supplemented broth II ( SPB II ) respectively , was compared .
	manualset3
147716	8	409687	5	NULL	NULL	0	NULL	 supplemented broth II ( SPB II ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of culturing 2 and 5 ml of blood in 18 ml of supplemented peptone broth I ( SPB I ) and 45 ml of supplemented broth II ( SPB II ) respectively , was compared .
	manualset3
147717	1	409688	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of dexamethasone administered intraperitoneally on hepatic glucocorticoid receptor binding capacity was measured in adrenalectomized male Swiss Webster mice .
	manualset3
147718	2	409688	5	NULL	NULL	0	NULL	dexamethasone 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of dexamethasone administered intraperitoneally on hepatic glucocorticoid receptor binding capacity was measured in adrenalectomized male Swiss Webster mice .
	manualset3
147719	3	409688	5	NULL	NULL	0	NULL	hepatic glucocorticoid receptor binding capacity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of dexamethasone administered intraperitoneally on hepatic glucocorticoid receptor binding capacity was measured in adrenalectomized male Swiss Webster mice .
	manualset3
147720	4	409688	5	NULL	NULL	0	NULL	adrenalectomized male Swiss Webster mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of dexamethasone administered intraperitoneally on hepatic glucocorticoid receptor binding capacity was measured in adrenalectomized male Swiss Webster mice .
	manualset3
147721	1	409689	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of dietary cholesterol and some lipid lowering agents .
	manualset3
147722	2	409689	5	NULL	NULL	0	NULL	dietary cholesterol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of dietary cholesterol and some lipid lowering agents .
	manualset3
147723	3	409689	5	NULL	NULL	0	NULL	lipid lowering agents	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of dietary cholesterol and some lipid lowering agents .
	manualset3
147724	1	409690	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of different Burkholderia pseudomallei isolates of varying levels of virulence on toll-like-receptor expression .
	manualset3
147725	2	409690	5	NULL	NULL	0	NULL	Burkholderia pseudomallei isolates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of different Burkholderia pseudomallei isolates of varying levels of virulence on toll-like-receptor expression .
	manualset3
147726	3	409690	5	NULL	NULL	0	NULL	varying levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of different Burkholderia pseudomallei isolates of varying levels of virulence on toll-like-receptor expression .
	manualset3
147727	4	409690	5	NULL	NULL	0	NULL	virulence 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of different Burkholderia pseudomallei isolates of varying levels of virulence on toll-like-receptor expression .
	manualset3
147728	5	409690	5	NULL	NULL	0	NULL	toll-like-receptor expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of different Burkholderia pseudomallei isolates of varying levels of virulence on toll-like-receptor expression .
	manualset3
147729	1	409691	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of different plasticizers , viz .
	manualset3
147730	2	409691	5	NULL	NULL	0	NULL	plasticizers 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of different plasticizers , viz .
	manualset3
147731	1	409692	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of dimercaprol on amine oxidase and amino acid decarboxylase of the normotensive and hypertensive rat kidney .
	manualset3
147732	2	409692	5	NULL	NULL	0	NULL	dimercaprol 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of dimercaprol on amine oxidase and amino acid decarboxylase of the normotensive and hypertensive rat kidney .
	manualset3
147733	3	409692	5	NULL	NULL	0	NULL	amine oxidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of dimercaprol on amine oxidase and amino acid decarboxylase of the normotensive and hypertensive rat kidney .
	manualset3
147734	4	409692	5	NULL	NULL	0	NULL	amino acid decarboxylase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of dimercaprol on amine oxidase and amino acid decarboxylase of the normotensive and hypertensive rat kidney .
	manualset3
147735	5	409692	5	NULL	NULL	0	NULL	normotensive rat kidney	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of dimercaprol on amine oxidase and amino acid decarboxylase of the normotensive and hypertensive rat kidney .
	manualset3
147736	6	409692	5	NULL	NULL	0	NULL	hypertensive rat kidney	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of dimercaprol on amine oxidase and amino acid decarboxylase of the normotensive and hypertensive rat kidney .
	manualset3
147737	1	409693	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of electroacupuncture on the function of sympatheto-adrenal medulla .
	manualset3
147738	2	409693	5	NULL	NULL	0	NULL	electroacupuncture 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of electroacupuncture on the function of sympatheto-adrenal medulla .
	manualset3
147739	3	409693	5	NULL	NULL	0	NULL	function 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of electroacupuncture on the function of sympatheto-adrenal medulla .
	manualset3
147740	4	409693	5	NULL	NULL	0	NULL	sympatheto-adrenal medulla	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of electroacupuncture on the function of sympatheto-adrenal medulla .
	manualset3
147741	1	409694	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of foreign anions along with primary ions on the performance of ion-selective electrode is investigated in terms of potentiometric selectivity coefficients , which were determined using the fixed interference method ( FIM ) at 1.0 x10 ( -2 ) M concentration of foreign anions .
	manualset3
147742	2	409694	5	NULL	NULL	0	NULL	foreign anions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of foreign anions along with primary ions on the performance of ion-selective electrode is investigated in terms of potentiometric selectivity coefficients , which were determined using the fixed interference method ( FIM ) at 1.0 x10 ( -2 ) M concentration of foreign anions .
	manualset3
147743	3	409694	5	NULL	NULL	0	NULL	primary ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of foreign anions along with primary ions on the performance of ion-selective electrode is investigated in terms of potentiometric selectivity coefficients , which were determined using the fixed interference method ( FIM ) at 1.0 x10 ( -2 ) M concentration of foreign anions .
	manualset3
147744	4	409694	5	NULL	NULL	0	NULL	performance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of foreign anions along with primary ions on the performance of ion-selective electrode is investigated in terms of potentiometric selectivity coefficients , which were determined using the fixed interference method ( FIM ) at 1.0 x10 ( -2 ) M concentration of foreign anions .
	manualset3
147745	5	409694	5	NULL	NULL	0	NULL	ion-selective electrode	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of foreign anions along with primary ions on the performance of ion-selective electrode is investigated in terms of potentiometric selectivity coefficients , which were determined using the fixed interference method ( FIM ) at 1.0 x10 ( -2 ) M concentration of foreign anions .
	manualset3
147746	6	409694	5	NULL	NULL	0	NULL	potentiometric selectivity coefficients	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of foreign anions along with primary ions on the performance of ion-selective electrode is investigated in terms of potentiometric selectivity coefficients , which were determined using the fixed interference method ( FIM ) at 1.0 x10 ( -2 ) M concentration of foreign anions .
	manualset3
147747	7	409694	5	NULL	NULL	0	NULL	fixed interference method ( FIM ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of foreign anions along with primary ions on the performance of ion-selective electrode is investigated in terms of potentiometric selectivity coefficients , which were determined using the fixed interference method ( FIM ) at 1.0 x10 ( -2 ) M concentration of foreign anions .
	manualset3
147748	8	409694	5	NULL	NULL	0	NULL	1.0 x10 ( -2 ) M concentration	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of foreign anions along with primary ions on the performance of ion-selective electrode is investigated in terms of potentiometric selectivity coefficients , which were determined using the fixed interference method ( FIM ) at 1.0 x10 ( -2 ) M concentration of foreign anions .
	manualset3
147749	9	409694	5	NULL	NULL	0	NULL	foreign anions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of foreign anions along with primary ions on the performance of ion-selective electrode is investigated in terms of potentiometric selectivity coefficients , which were determined using the fixed interference method ( FIM ) at 1.0 x10 ( -2 ) M concentration of foreign anions .
	manualset3
147750	1	409695	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of four neuropeptides and acetylcholine on the release of leukotrienes LTC4 , LTD4 and LTE4 from platelet activating factor-stimulated rat lung and ionophore A23187-stimulated guinea pig lung , as detected by the combined use of HPLC and radioimmunoassay , was studied .
	manualset3
147751	2	409695	5	NULL	NULL	0	NULL	four 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of four neuropeptides and acetylcholine on the release of leukotrienes LTC4 , LTD4 and LTE4 from platelet activating factor-stimulated rat lung and ionophore A23187-stimulated guinea pig lung , as detected by the combined use of HPLC and radioimmunoassay , was studied .
	manualset3
147752	3	409695	5	NULL	NULL	0	NULL	neuropeptides 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of four neuropeptides and acetylcholine on the release of leukotrienes LTC4 , LTD4 and LTE4 from platelet activating factor-stimulated rat lung and ionophore A23187-stimulated guinea pig lung , as detected by the combined use of HPLC and radioimmunoassay , was studied .
	manualset3
147753	4	409695	5	NULL	NULL	0	NULL	acetylcholine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of four neuropeptides and acetylcholine on the release of leukotrienes LTC4 , LTD4 and LTE4 from platelet activating factor-stimulated rat lung and ionophore A23187-stimulated guinea pig lung , as detected by the combined use of HPLC and radioimmunoassay , was studied .
	manualset3
147754	5	409695	5	NULL	NULL	0	NULL	release 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of four neuropeptides and acetylcholine on the release of leukotrienes LTC4 , LTD4 and LTE4 from platelet activating factor-stimulated rat lung and ionophore A23187-stimulated guinea pig lung , as detected by the combined use of HPLC and radioimmunoassay , was studied .
	manualset3
147755	6	409695	5	NULL	NULL	0	NULL	leukotriene LTC4 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of four neuropeptides and acetylcholine on the release of leukotrienes LTC4 , LTD4 and LTE4 from platelet activating factor-stimulated rat lung and ionophore A23187-stimulated guinea pig lung , as detected by the combined use of HPLC and radioimmunoassay , was studied .
	manualset3
147756	7	409695	5	NULL	NULL	0	NULL	leukotriene LTD4 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of four neuropeptides and acetylcholine on the release of leukotrienes LTC4 , LTD4 and LTE4 from platelet activating factor-stimulated rat lung and ionophore A23187-stimulated guinea pig lung , as detected by the combined use of HPLC and radioimmunoassay , was studied .
	manualset3
147757	8	409695	5	NULL	NULL	0	NULL	leukotriene LTE4 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of four neuropeptides and acetylcholine on the release of leukotrienes LTC4 , LTD4 and LTE4 from platelet activating factor-stimulated rat lung and ionophore A23187-stimulated guinea pig lung , as detected by the combined use of HPLC and radioimmunoassay , was studied .
	manualset3
147758	9	409695	5	NULL	NULL	0	NULL	platelet activating factor-stimulated rat lung	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of four neuropeptides and acetylcholine on the release of leukotrienes LTC4 , LTD4 and LTE4 from platelet activating factor-stimulated rat lung and ionophore A23187-stimulated guinea pig lung , as detected by the combined use of HPLC and radioimmunoassay , was studied .
	manualset3
147759	10	409695	5	NULL	NULL	0	NULL	ionophore A23187-stimulated guinea pig lung 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of four neuropeptides and acetylcholine on the release of leukotrienes LTC4 , LTD4 and LTE4 from platelet activating factor-stimulated rat lung and ionophore A23187-stimulated guinea pig lung , as detected by the combined use of HPLC and radioimmunoassay , was studied .
	manualset3
147760	11	409695	5	NULL	NULL	0	NULL	combined use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of four neuropeptides and acetylcholine on the release of leukotrienes LTC4 , LTD4 and LTE4 from platelet activating factor-stimulated rat lung and ionophore A23187-stimulated guinea pig lung , as detected by the combined use of HPLC and radioimmunoassay , was studied .
	manualset3
147761	12	409695	5	NULL	NULL	0	NULL	HPLC 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of four neuropeptides and acetylcholine on the release of leukotrienes LTC4 , LTD4 and LTE4 from platelet activating factor-stimulated rat lung and ionophore A23187-stimulated guinea pig lung , as detected by the combined use of HPLC and radioimmunoassay , was studied .
	manualset3
147762	13	409695	5	NULL	NULL	0	NULL	radioimmunoassay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of four neuropeptides and acetylcholine on the release of leukotrienes LTC4 , LTD4 and LTE4 from platelet activating factor-stimulated rat lung and ionophore A23187-stimulated guinea pig lung , as detected by the combined use of HPLC and radioimmunoassay , was studied .
	manualset3
147763	1	409696	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of glutaraldehyde ( the active component of `` UrinAid '' ) on Syva EMIT II drugs-of-abuse screening assays was studied .
	manualset3
147764	2	409696	5	NULL	NULL	NULL	NULL	glutaraldehyde ( the active component of `` UrinAid '' ) 	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The effect of glutaraldehyde ( the active component of `` UrinAid '' ) on Syva EMIT II drugs-of-abuse screening assays was studied .
	manualset3
147765	3	409696	5	NULL	NULL	0	NULL	Syva EMIT II drugs-of-abuse screening assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of glutaraldehyde ( the active component of `` UrinAid '' ) on Syva EMIT II drugs-of-abuse screening assays was studied .
	manualset3
147766	1	409697	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of glycerol disappeared with high levels of dietary protein , whereas the effects of lactate and pyruvate disappeared with high levels of dietary fat .
	manualset3
147767	2	409697	5	NULL	NULL	0	NULL	glycerol 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of glycerol disappeared with high levels of dietary protein , whereas the effects of lactate and pyruvate disappeared with high levels of dietary fat .
	manualset3
147768	3	409697	5	NULL	NULL	0	NULL	high levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of glycerol disappeared with high levels of dietary protein , whereas the effects of lactate and pyruvate disappeared with high levels of dietary fat .
	manualset3
147769	4	409697	5	NULL	NULL	0	NULL	dietary protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of glycerol disappeared with high levels of dietary protein , whereas the effects of lactate and pyruvate disappeared with high levels of dietary fat .
	manualset3
147770	5	409697	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of glycerol disappeared with high levels of dietary protein , whereas the effects of lactate and pyruvate disappeared with high levels of dietary fat .
	manualset3
147771	6	409697	5	NULL	NULL	0	NULL	lactate 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of glycerol disappeared with high levels of dietary protein , whereas the effects of lactate and pyruvate disappeared with high levels of dietary fat .
	manualset3
147772	7	409697	5	NULL	NULL	0	NULL	pyruvate 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of glycerol disappeared with high levels of dietary protein , whereas the effects of lactate and pyruvate disappeared with high levels of dietary fat .
	manualset3
147773	8	409697	5	NULL	NULL	0	NULL	high levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of glycerol disappeared with high levels of dietary protein , whereas the effects of lactate and pyruvate disappeared with high levels of dietary fat .
	manualset3
147774	9	409697	5	NULL	NULL	0	NULL	dietary fat	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of glycerol disappeared with high levels of dietary protein , whereas the effects of lactate and pyruvate disappeared with high levels of dietary fat .
	manualset3
147775	1	409698	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of growth medium salinity of Photobacterium damselae subsp .
	manualset3
147776	2	409698	5	NULL	NULL	0	NULL	growth medium salinity 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of growth medium salinity of Photobacterium damselae subsp .
	manualset3
147777	3	409698	5	NULL	NULL	0	NULL	Photobacterium damselae subsp	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of growth medium salinity of Photobacterium damselae subsp .
	manualset3
147778	1	409699	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of hallux valgus correction on chronic plantar ulceration .
	manualset3
147779	2	409699	5	NULL	NULL	0	NULL	hallux valgus correction	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of hallux valgus correction on chronic plantar ulceration .
	manualset3
147780	3	409699	5	NULL	NULL	0	NULL	chronic plantar ulceration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of hallux valgus correction on chronic plantar ulceration .
	manualset3
147781	1	409700	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of head and neck cancer treatment on whole salivary flow .
	manualset3
147782	2	409700	5	NULL	NULL	0	NULL	head and neck cancer treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of head and neck cancer treatment on whole salivary flow .
	manualset3
147783	3	409700	5	NULL	NULL	0	NULL	salivary flow	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of head and neck cancer treatment on whole salivary flow .
	manualset3
147784	1	409701	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of helper phages and -- or multiplicity of infection on the repair of ultraviolet damages in T4 .
	manualset3
147785	2	409701	5	NULL	NULL	0	NULL	helper phages	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of helper phages and -- or multiplicity of infection on the repair of ultraviolet damages in T4 .
	manualset3
147786	3	409701	5	NULL	NULL	NULL	NULL	multiplicity of infection 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The effect of helper phages and -- or multiplicity of infection on the repair of ultraviolet damages in T4 .
	manualset3
147787	4	409701	5	NULL	NULL	0	NULL	repair 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of helper phages and -- or multiplicity of infection on the repair of ultraviolet damages in T4 .
	manualset3
147788	5	409701	5	NULL	NULL	0	NULL	ultraviolet damages	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of helper phages and -- or multiplicity of infection on the repair of ultraviolet damages in T4 .
	manualset3
147789	6	409701	5	NULL	NULL	0	NULL	T4 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of helper phages and -- or multiplicity of infection on the repair of ultraviolet damages in T4 .
	manualset3
147790	1	409702	5	NULL	NULL	0	NULL	spectrum 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A spectrum of adverse drug reactions that are caused by the combined action of drugs and viruses has been described : ampicillin rash in acute infectious mononucleosis ; Reye 's syndrome ; hypersensitivity reactions to sulphonamides in patients with HIV infection ; drug-induced agranulocytosis ; paracetamol ( acetaminophen ) hepatotoxicity ; aspirin ( acetylsalicyclic acid ) - induced asthma ; Epstein-Barr virus-associated lymphoma and methotrexate ; and AIDS-related Kaposi 's sarcoma and nitrite use .
	manualset3
147791	2	409702	5	NULL	NULL	0	NULL	adverse drug reactions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A spectrum of adverse drug reactions that are caused by the combined action of drugs and viruses has been described : ampicillin rash in acute infectious mononucleosis ; Reye 's syndrome ; hypersensitivity reactions to sulphonamides in patients with HIV infection ; drug-induced agranulocytosis ; paracetamol ( acetaminophen ) hepatotoxicity ; aspirin ( acetylsalicyclic acid ) - induced asthma ; Epstein-Barr virus-associated lymphoma and methotrexate ; and AIDS-related Kaposi 's sarcoma and nitrite use .
	manualset3
147792	3	409702	5	NULL	NULL	0	NULL	combined action 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A spectrum of adverse drug reactions that are caused by the combined action of drugs and viruses has been described : ampicillin rash in acute infectious mononucleosis ; Reye 's syndrome ; hypersensitivity reactions to sulphonamides in patients with HIV infection ; drug-induced agranulocytosis ; paracetamol ( acetaminophen ) hepatotoxicity ; aspirin ( acetylsalicyclic acid ) - induced asthma ; Epstein-Barr virus-associated lymphoma and methotrexate ; and AIDS-related Kaposi 's sarcoma and nitrite use .
	manualset3
147793	4	409702	5	NULL	NULL	0	NULL	drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A spectrum of adverse drug reactions that are caused by the combined action of drugs and viruses has been described : ampicillin rash in acute infectious mononucleosis ; Reye 's syndrome ; hypersensitivity reactions to sulphonamides in patients with HIV infection ; drug-induced agranulocytosis ; paracetamol ( acetaminophen ) hepatotoxicity ; aspirin ( acetylsalicyclic acid ) - induced asthma ; Epstein-Barr virus-associated lymphoma and methotrexate ; and AIDS-related Kaposi 's sarcoma and nitrite use .
	manualset3
147794	5	409702	5	NULL	NULL	0	NULL	viruses 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A spectrum of adverse drug reactions that are caused by the combined action of drugs and viruses has been described : ampicillin rash in acute infectious mononucleosis ; Reye 's syndrome ; hypersensitivity reactions to sulphonamides in patients with HIV infection ; drug-induced agranulocytosis ; paracetamol ( acetaminophen ) hepatotoxicity ; aspirin ( acetylsalicyclic acid ) - induced asthma ; Epstein-Barr virus-associated lymphoma and methotrexate ; and AIDS-related Kaposi 's sarcoma and nitrite use .
	manualset3
147795	6	409702	5	NULL	NULL	0	NULL	ampicillin rash 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A spectrum of adverse drug reactions that are caused by the combined action of drugs and viruses has been described : ampicillin rash in acute infectious mononucleosis ; Reye 's syndrome ; hypersensitivity reactions to sulphonamides in patients with HIV infection ; drug-induced agranulocytosis ; paracetamol ( acetaminophen ) hepatotoxicity ; aspirin ( acetylsalicyclic acid ) - induced asthma ; Epstein-Barr virus-associated lymphoma and methotrexate ; and AIDS-related Kaposi 's sarcoma and nitrite use .
	manualset3
147796	7	409702	5	NULL	NULL	0	NULL	acute infectious mononucleosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A spectrum of adverse drug reactions that are caused by the combined action of drugs and viruses has been described : ampicillin rash in acute infectious mononucleosis ; Reye 's syndrome ; hypersensitivity reactions to sulphonamides in patients with HIV infection ; drug-induced agranulocytosis ; paracetamol ( acetaminophen ) hepatotoxicity ; aspirin ( acetylsalicyclic acid ) - induced asthma ; Epstein-Barr virus-associated lymphoma and methotrexate ; and AIDS-related Kaposi 's sarcoma and nitrite use .
	manualset3
147797	8	409702	5	NULL	NULL	0	NULL	Reye 's syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A spectrum of adverse drug reactions that are caused by the combined action of drugs and viruses has been described : ampicillin rash in acute infectious mononucleosis ; Reye 's syndrome ; hypersensitivity reactions to sulphonamides in patients with HIV infection ; drug-induced agranulocytosis ; paracetamol ( acetaminophen ) hepatotoxicity ; aspirin ( acetylsalicyclic acid ) - induced asthma ; Epstein-Barr virus-associated lymphoma and methotrexate ; and AIDS-related Kaposi 's sarcoma and nitrite use .
	manualset3
147798	9	409702	5	NULL	NULL	0	NULL	hypersensitivity reactions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A spectrum of adverse drug reactions that are caused by the combined action of drugs and viruses has been described : ampicillin rash in acute infectious mononucleosis ; Reye 's syndrome ; hypersensitivity reactions to sulphonamides in patients with HIV infection ; drug-induced agranulocytosis ; paracetamol ( acetaminophen ) hepatotoxicity ; aspirin ( acetylsalicyclic acid ) - induced asthma ; Epstein-Barr virus-associated lymphoma and methotrexate ; and AIDS-related Kaposi 's sarcoma and nitrite use .
	manualset3
147799	10	409702	5	NULL	NULL	0	NULL	sulphonamides 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A spectrum of adverse drug reactions that are caused by the combined action of drugs and viruses has been described : ampicillin rash in acute infectious mononucleosis ; Reye 's syndrome ; hypersensitivity reactions to sulphonamides in patients with HIV infection ; drug-induced agranulocytosis ; paracetamol ( acetaminophen ) hepatotoxicity ; aspirin ( acetylsalicyclic acid ) - induced asthma ; Epstein-Barr virus-associated lymphoma and methotrexate ; and AIDS-related Kaposi 's sarcoma and nitrite use .
	manualset3
147800	11	409702	5	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A spectrum of adverse drug reactions that are caused by the combined action of drugs and viruses has been described : ampicillin rash in acute infectious mononucleosis ; Reye 's syndrome ; hypersensitivity reactions to sulphonamides in patients with HIV infection ; drug-induced agranulocytosis ; paracetamol ( acetaminophen ) hepatotoxicity ; aspirin ( acetylsalicyclic acid ) - induced asthma ; Epstein-Barr virus-associated lymphoma and methotrexate ; and AIDS-related Kaposi 's sarcoma and nitrite use .
	manualset3
147801	12	409702	5	NULL	NULL	0	NULL	HIV infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A spectrum of adverse drug reactions that are caused by the combined action of drugs and viruses has been described : ampicillin rash in acute infectious mononucleosis ; Reye 's syndrome ; hypersensitivity reactions to sulphonamides in patients with HIV infection ; drug-induced agranulocytosis ; paracetamol ( acetaminophen ) hepatotoxicity ; aspirin ( acetylsalicyclic acid ) - induced asthma ; Epstein-Barr virus-associated lymphoma and methotrexate ; and AIDS-related Kaposi 's sarcoma and nitrite use .
	manualset3
147802	13	409702	5	NULL	NULL	0	NULL	drug-induced agranulocytosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A spectrum of adverse drug reactions that are caused by the combined action of drugs and viruses has been described : ampicillin rash in acute infectious mononucleosis ; Reye 's syndrome ; hypersensitivity reactions to sulphonamides in patients with HIV infection ; drug-induced agranulocytosis ; paracetamol ( acetaminophen ) hepatotoxicity ; aspirin ( acetylsalicyclic acid ) - induced asthma ; Epstein-Barr virus-associated lymphoma and methotrexate ; and AIDS-related Kaposi 's sarcoma and nitrite use .
	manualset3
147803	14	409702	5	NULL	NULL	0	NULL	paracetamol ( acetaminophen ) hepatotoxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A spectrum of adverse drug reactions that are caused by the combined action of drugs and viruses has been described : ampicillin rash in acute infectious mononucleosis ; Reye 's syndrome ; hypersensitivity reactions to sulphonamides in patients with HIV infection ; drug-induced agranulocytosis ; paracetamol ( acetaminophen ) hepatotoxicity ; aspirin ( acetylsalicyclic acid ) - induced asthma ; Epstein-Barr virus-associated lymphoma and methotrexate ; and AIDS-related Kaposi 's sarcoma and nitrite use .
	manualset3
147804	15	409702	5	NULL	NULL	0	NULL	aspirin ( acetylsalicyclic acid ) - induced asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A spectrum of adverse drug reactions that are caused by the combined action of drugs and viruses has been described : ampicillin rash in acute infectious mononucleosis ; Reye 's syndrome ; hypersensitivity reactions to sulphonamides in patients with HIV infection ; drug-induced agranulocytosis ; paracetamol ( acetaminophen ) hepatotoxicity ; aspirin ( acetylsalicyclic acid ) - induced asthma ; Epstein-Barr virus-associated lymphoma and methotrexate ; and AIDS-related Kaposi 's sarcoma and nitrite use .
	manualset3
147805	16	409702	5	NULL	NULL	0	NULL	Epstein-Barr virus-associated lymphoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A spectrum of adverse drug reactions that are caused by the combined action of drugs and viruses has been described : ampicillin rash in acute infectious mononucleosis ; Reye 's syndrome ; hypersensitivity reactions to sulphonamides in patients with HIV infection ; drug-induced agranulocytosis ; paracetamol ( acetaminophen ) hepatotoxicity ; aspirin ( acetylsalicyclic acid ) - induced asthma ; Epstein-Barr virus-associated lymphoma and methotrexate ; and AIDS-related Kaposi 's sarcoma and nitrite use .
	manualset3
147806	17	409702	5	NULL	NULL	0	NULL	methotrexate 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A spectrum of adverse drug reactions that are caused by the combined action of drugs and viruses has been described : ampicillin rash in acute infectious mononucleosis ; Reye 's syndrome ; hypersensitivity reactions to sulphonamides in patients with HIV infection ; drug-induced agranulocytosis ; paracetamol ( acetaminophen ) hepatotoxicity ; aspirin ( acetylsalicyclic acid ) - induced asthma ; Epstein-Barr virus-associated lymphoma and methotrexate ; and AIDS-related Kaposi 's sarcoma and nitrite use .
	manualset3
147807	18	409702	5	NULL	NULL	0	NULL	AIDS-related Kaposi 's sarcoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A spectrum of adverse drug reactions that are caused by the combined action of drugs and viruses has been described : ampicillin rash in acute infectious mononucleosis ; Reye 's syndrome ; hypersensitivity reactions to sulphonamides in patients with HIV infection ; drug-induced agranulocytosis ; paracetamol ( acetaminophen ) hepatotoxicity ; aspirin ( acetylsalicyclic acid ) - induced asthma ; Epstein-Barr virus-associated lymphoma and methotrexate ; and AIDS-related Kaposi 's sarcoma and nitrite use .
	manualset3
147808	19	409702	5	NULL	NULL	0	NULL	nitrite use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A spectrum of adverse drug reactions that are caused by the combined action of drugs and viruses has been described : ampicillin rash in acute infectious mononucleosis ; Reye 's syndrome ; hypersensitivity reactions to sulphonamides in patients with HIV infection ; drug-induced agranulocytosis ; paracetamol ( acetaminophen ) hepatotoxicity ; aspirin ( acetylsalicyclic acid ) - induced asthma ; Epstein-Barr virus-associated lymphoma and methotrexate ; and AIDS-related Kaposi 's sarcoma and nitrite use .
	manualset3
147809	1	409703	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of hydrogen ion concentration on the precipitating and protective actions of proteins on colloidal gold and gum benzoin .
	manualset3
147810	2	409703	5	NULL	NULL	0	NULL	hydrogen ion concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of hydrogen ion concentration on the precipitating and protective actions of proteins on colloidal gold and gum benzoin .
	manualset3
147811	3	409703	5	NULL	NULL	0	NULL	precipitating action	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of hydrogen ion concentration on the precipitating and protective actions of proteins on colloidal gold and gum benzoin .
	manualset3
147812	4	409703	5	NULL	NULL	0	NULL	protective actions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of hydrogen ion concentration on the precipitating and protective actions of proteins on colloidal gold and gum benzoin .
	manualset3
147813	5	409703	5	NULL	NULL	0	NULL	proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of hydrogen ion concentration on the precipitating and protective actions of proteins on colloidal gold and gum benzoin .
	manualset3
147814	6	409703	5	NULL	NULL	0	NULL	colloidal gold	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of hydrogen ion concentration on the precipitating and protective actions of proteins on colloidal gold and gum benzoin .
	manualset3
147815	7	409703	5	NULL	NULL	0	NULL	gum benzoin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of hydrogen ion concentration on the precipitating and protective actions of proteins on colloidal gold and gum benzoin .
	manualset3
147816	1	409704	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of hypoalbuminemia , hyperbilirubinemia and renal failure on serum fructosamine concentration in non-diabetic individuals .
	manualset3
147817	2	409704	5	NULL	NULL	0	NULL	hypoalbuminemia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of hypoalbuminemia , hyperbilirubinemia and renal failure on serum fructosamine concentration in non-diabetic individuals .
	manualset3
147818	3	409704	5	NULL	NULL	0	NULL	hyperbilirubinemia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of hypoalbuminemia , hyperbilirubinemia and renal failure on serum fructosamine concentration in non-diabetic individuals .
	manualset3
147819	4	409704	5	NULL	NULL	0	NULL	renal failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of hypoalbuminemia , hyperbilirubinemia and renal failure on serum fructosamine concentration in non-diabetic individuals .
	manualset3
147820	5	409704	5	NULL	NULL	0	NULL	serum fructosamine concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of hypoalbuminemia , hyperbilirubinemia and renal failure on serum fructosamine concentration in non-diabetic individuals .
	manualset3
147821	6	409704	5	NULL	NULL	0	NULL	non-diabetic individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of hypoalbuminemia , hyperbilirubinemia and renal failure on serum fructosamine concentration in non-diabetic individuals .
	manualset3
147822	1	409705	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of impurities on the chemotherapeutic action of crystalline penicillin .
	manualset3
147823	2	409705	5	NULL	NULL	0	NULL	impurities 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of impurities on the chemotherapeutic action of crystalline penicillin .
	manualset3
147824	3	409705	5	NULL	NULL	0	NULL	chemotherapeutic action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of impurities on the chemotherapeutic action of crystalline penicillin .
	manualset3
147825	4	409705	5	NULL	NULL	0	NULL	crystalline penicillin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of impurities on the chemotherapeutic action of crystalline penicillin .
	manualset3
147826	1	409706	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of induction method on defibrillation threshold and ventricular fibrillation cycle length .
	manualset3
147827	2	409706	5	NULL	NULL	0	NULL	induction method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of induction method on defibrillation threshold and ventricular fibrillation cycle length .
	manualset3
147828	3	409706	5	NULL	NULL	0	NULL	defibrillation threshold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of induction method on defibrillation threshold and ventricular fibrillation cycle length .
	manualset3
147829	4	409706	5	NULL	NULL	0	NULL	ventricular fibrillation cycle length	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of induction method on defibrillation threshold and ventricular fibrillation cycle length .
	manualset3
147830	1	409707	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of inorganic phosphate on Ca2 + retention has been investigated using phosphate-depleted liver mitchondria .
	manualset3
147831	2	409707	5	NULL	NULL	0	NULL	inorganic phosphate	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of inorganic phosphate on Ca2 + retention has been investigated using phosphate-depleted liver mitchondria .
	manualset3
147832	3	409707	5	NULL	NULL	0	NULL	Ca2 + retention	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of inorganic phosphate on Ca2 + retention has been investigated using phosphate-depleted liver mitchondria .
	manualset3
147833	4	409707	5	NULL	NULL	0	NULL	phosphate-depleted liver mitchondria	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of inorganic phosphate on Ca2 + retention has been investigated using phosphate-depleted liver mitchondria .
	manualset3
147834	1	409708	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of intravenous heparin and mepesulfate on cholesterol partition and the lipoprotein pattern .
	manualset3
147835	2	409708	5	NULL	NULL	0	NULL	intravenous heparin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of intravenous heparin and mepesulfate on cholesterol partition and the lipoprotein pattern .
	manualset3
147836	3	409708	5	NULL	NULL	0	NULL	mepesulfate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of intravenous heparin and mepesulfate on cholesterol partition and the lipoprotein pattern .
	manualset3
147837	4	409708	5	NULL	NULL	0	NULL	cholesterol partition	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of intravenous heparin and mepesulfate on cholesterol partition and the lipoprotein pattern .
	manualset3
147838	5	409708	5	NULL	NULL	0	NULL	lipoprotein pattern	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of intravenous heparin and mepesulfate on cholesterol partition and the lipoprotein pattern .
	manualset3
147839	1	409709	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of lipophilic compounds upon the activity of rat liver mitochondrial monoamine oxidase-A and - B .
	manualset3
147840	2	409709	5	NULL	NULL	0	NULL	lipophilic compounds 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of lipophilic compounds upon the activity of rat liver mitochondrial monoamine oxidase-A and - B .
	manualset3
147841	3	409709	5	NULL	NULL	0	NULL	activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of lipophilic compounds upon the activity of rat liver mitochondrial monoamine oxidase-A and - B .
	manualset3
147842	4	409709	5	NULL	NULL	0	NULL	rat liver mitochondrial monoamine oxidase-A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of lipophilic compounds upon the activity of rat liver mitochondrial monoamine oxidase-A and - B .
	manualset3
147843	5	409709	5	NULL	NULL	0	NULL	rat liver mitochondrial monoamine oxidase-B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of lipophilic compounds upon the activity of rat liver mitochondrial monoamine oxidase-A and - B .
	manualset3
147844	1	409710	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of oxygen at high pressure ( OHP ) on resting membrane properties ( effective membrane resistance ( Reff ) and membrane potential ( Vm ) ) and the spontaneous release of excitatory transmitter were examined at the lobster neuromuscular junction .
	manualset3
147845	2	409710	5	NULL	NULL	0	NULL	oxygen at high pressure ( OHP )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of oxygen at high pressure ( OHP ) on resting membrane properties ( effective membrane resistance ( Reff ) and membrane potential ( Vm ) ) and the spontaneous release of excitatory transmitter were examined at the lobster neuromuscular junction .
	manualset3
147846	3	409710	5	NULL	NULL	0	NULL	resting membrane properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of oxygen at high pressure ( OHP ) on resting membrane properties ( effective membrane resistance ( Reff ) and membrane potential ( Vm ) ) and the spontaneous release of excitatory transmitter were examined at the lobster neuromuscular junction .
	manualset3
147847	4	409710	5	NULL	NULL	0	NULL	effective membrane resistance ( Reff ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of oxygen at high pressure ( OHP ) on resting membrane properties ( effective membrane resistance ( Reff ) and membrane potential ( Vm ) ) and the spontaneous release of excitatory transmitter were examined at the lobster neuromuscular junction .
	manualset3
147848	5	409710	5	NULL	NULL	0	NULL	membrane potential ( Vm )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of oxygen at high pressure ( OHP ) on resting membrane properties ( effective membrane resistance ( Reff ) and membrane potential ( Vm ) ) and the spontaneous release of excitatory transmitter were examined at the lobster neuromuscular junction .
	manualset3
147849	6	409710	5	NULL	NULL	0	NULL	spontaneous release	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of oxygen at high pressure ( OHP ) on resting membrane properties ( effective membrane resistance ( Reff ) and membrane potential ( Vm ) ) and the spontaneous release of excitatory transmitter were examined at the lobster neuromuscular junction .
	manualset3
147850	7	409710	5	NULL	NULL	0	NULL	excitatory transmitter	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of oxygen at high pressure ( OHP ) on resting membrane properties ( effective membrane resistance ( Reff ) and membrane potential ( Vm ) ) and the spontaneous release of excitatory transmitter were examined at the lobster neuromuscular junction .
	manualset3
147851	8	409710	5	NULL	NULL	0	NULL	lobster neuromuscular junction 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of oxygen at high pressure ( OHP ) on resting membrane properties ( effective membrane resistance ( Reff ) and membrane potential ( Vm ) ) and the spontaneous release of excitatory transmitter were examined at the lobster neuromuscular junction .
	manualset3
147852	1	409711	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of parenteral lipid emulsion-induced hyperlipidemia on prostaglandin E1 modulation of platelet function .
	manualset3
147853	2	409711	5	NULL	NULL	0	NULL	parenteral lipid emulsion-induced hyperlipidemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of parenteral lipid emulsion-induced hyperlipidemia on prostaglandin E1 modulation of platelet function .
	manualset3
147854	3	409711	5	NULL	NULL	0	NULL	prostaglandin E1 modulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of parenteral lipid emulsion-induced hyperlipidemia on prostaglandin E1 modulation of platelet function .
	manualset3
147855	4	409711	5	NULL	NULL	0	NULL	platelet function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of parenteral lipid emulsion-induced hyperlipidemia on prostaglandin E1 modulation of platelet function .
	manualset3
147856	1	409712	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of periprocedure chemotherapy has not been established .
	manualset3
147857	2	409712	5	NULL	NULL	0	NULL	periprocedure chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of periprocedure chemotherapy has not been established .
	manualset3
147858	1	409713	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of polyamines ( putrescine , spermine , and spermidine ) on the oxidation of exogenous NADH by Jerusalem artichoke ( Helianthus tuberosus L. cv .
	manualset3
147859	2	409713	5	NULL	NULL	0	NULL	polyamines 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of polyamines ( putrescine , spermine , and spermidine ) on the oxidation of exogenous NADH by Jerusalem artichoke ( Helianthus tuberosus L. cv .
	manualset3
147860	3	409713	5	NULL	NULL	0	NULL	putrescine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of polyamines ( putrescine , spermine , and spermidine ) on the oxidation of exogenous NADH by Jerusalem artichoke ( Helianthus tuberosus L. cv .
	manualset3
147861	4	409713	5	NULL	NULL	0	NULL	spermine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of polyamines ( putrescine , spermine , and spermidine ) on the oxidation of exogenous NADH by Jerusalem artichoke ( Helianthus tuberosus L. cv .
	manualset3
147862	5	409713	5	NULL	NULL	0	NULL	spermidine 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of polyamines ( putrescine , spermine , and spermidine ) on the oxidation of exogenous NADH by Jerusalem artichoke ( Helianthus tuberosus L. cv .
	manualset3
147863	6	409713	5	NULL	NULL	0	NULL	oxidation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of polyamines ( putrescine , spermine , and spermidine ) on the oxidation of exogenous NADH by Jerusalem artichoke ( Helianthus tuberosus L. cv .
	manualset3
147864	7	409713	5	NULL	NULL	0	NULL	exogenous NADH	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of polyamines ( putrescine , spermine , and spermidine ) on the oxidation of exogenous NADH by Jerusalem artichoke ( Helianthus tuberosus L. cv .
	manualset3
147865	8	409713	5	NULL	NULL	0	NULL	Jerusalem artichoke ( Helianthus tuberosus L. cv 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of polyamines ( putrescine , spermine , and spermidine ) on the oxidation of exogenous NADH by Jerusalem artichoke ( Helianthus tuberosus L. cv .
	manualset3
147866	1	409714	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of practice on recall of negative material in dysphoria .
	manualset3
147867	2	409714	5	NULL	NULL	0	NULL	practice 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of practice on recall of negative material in dysphoria .
	manualset3
147868	3	409714	5	NULL	NULL	0	NULL	recall 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of practice on recall of negative material in dysphoria .
	manualset3
147869	4	409714	5	NULL	NULL	0	NULL	negative material	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of practice on recall of negative material in dysphoria .
	manualset3
147870	5	409714	5	NULL	NULL	0	NULL	dysphoria 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of practice on recall of negative material in dysphoria .
	manualset3
147871	1	409715	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of purified human plasma fibronectin ( FN ) on the reactivity of human lymphocyte-rich mononuclear cells to mitogens and allogeneic cell interactions was studied .
	manualset3
147872	2	409715	5	NULL	NULL	0	NULL	purified human plasma fibronectin ( FN )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of purified human plasma fibronectin ( FN ) on the reactivity of human lymphocyte-rich mononuclear cells to mitogens and allogeneic cell interactions was studied .
	manualset3
147873	3	409715	5	NULL	NULL	0	NULL	reactivity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of purified human plasma fibronectin ( FN ) on the reactivity of human lymphocyte-rich mononuclear cells to mitogens and allogeneic cell interactions was studied .
	manualset3
147874	4	409715	5	NULL	NULL	0	NULL	human lymphocyte-rich mononuclear cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of purified human plasma fibronectin ( FN ) on the reactivity of human lymphocyte-rich mononuclear cells to mitogens and allogeneic cell interactions was studied .
	manualset3
147875	5	409715	5	NULL	NULL	0	NULL	mitogens 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of purified human plasma fibronectin ( FN ) on the reactivity of human lymphocyte-rich mononuclear cells to mitogens and allogeneic cell interactions was studied .
	manualset3
147876	6	409715	5	NULL	NULL	0	NULL	allogeneic cell interactions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of purified human plasma fibronectin ( FN ) on the reactivity of human lymphocyte-rich mononuclear cells to mitogens and allogeneic cell interactions was studied .
	manualset3
147877	1	409716	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of rebreathing CO2 on ventilation and diaphragmatic electromyography in newborn infants .
	manualset3
147878	2	409716	5	NULL	NULL	0	NULL	CO2 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of rebreathing CO2 on ventilation and diaphragmatic electromyography in newborn infants .
	manualset3
147879	3	409716	5	NULL	NULL	0	NULL	ventilation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of rebreathing CO2 on ventilation and diaphragmatic electromyography in newborn infants .
	manualset3
147880	4	409716	5	NULL	NULL	0	NULL	diaphragmatic electromyography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of rebreathing CO2 on ventilation and diaphragmatic electromyography in newborn infants .
	manualset3
147881	5	409716	5	NULL	NULL	0	NULL	newborn infants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of rebreathing CO2 on ventilation and diaphragmatic electromyography in newborn infants .
	manualset3
147882	1	409717	5	NULL	NULL	0	NULL	stable integration vector	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A stable integration vector containing attP and int was constructed , and integration in L. lactis subsp .
	manualset3
147883	2	409717	5	NULL	NULL	0	NULL	attP 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A stable integration vector containing attP and int was constructed , and integration in L. lactis subsp .
	manualset3
147884	3	409717	5	NULL	NULL	0	NULL	int 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A stable integration vector containing attP and int was constructed , and integration in L. lactis subsp .
	manualset3
147885	4	409717	5	NULL	NULL	0	NULL	integration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A stable integration vector containing attP and int was constructed , and integration in L. lactis subsp .
	manualset3
147886	5	409717	5	NULL	NULL	0	NULL	L. lactis subsp	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A stable integration vector containing attP and int was constructed , and integration in L. lactis subsp .
	manualset3
147887	1	409718	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of renal failure on the disposition and neuromuscular blocking action of pancuronium bromide .
	manualset3
147888	2	409718	5	NULL	NULL	0	NULL	renal failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of renal failure on the disposition and neuromuscular blocking action of pancuronium bromide .
	manualset3
147889	3	409718	5	NULL	NULL	0	NULL	disposition 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of renal failure on the disposition and neuromuscular blocking action of pancuronium bromide .
	manualset3
147890	4	409718	5	NULL	NULL	0	NULL	neuromuscular blocking action 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of renal failure on the disposition and neuromuscular blocking action of pancuronium bromide .
	manualset3
147891	5	409718	5	NULL	NULL	0	NULL	pancuronium bromide	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of renal failure on the disposition and neuromuscular blocking action of pancuronium bromide .
	manualset3
147892	1	409719	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of ristomycin , chloramphenicol , kanamycin , benzylpenicillin , streptomycin , and cephaloridine on the indices of cellular and humoral immunity was studied comparatively on intact animals and on animals with secondary immune deficiency .
	manualset3
147893	2	409719	5	NULL	NULL	0	NULL	ristomycin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of ristomycin , chloramphenicol , kanamycin , benzylpenicillin , streptomycin , and cephaloridine on the indices of cellular and humoral immunity was studied comparatively on intact animals and on animals with secondary immune deficiency .
	manualset3
147894	3	409719	5	NULL	NULL	0	NULL	chloramphenicol 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of ristomycin , chloramphenicol , kanamycin , benzylpenicillin , streptomycin , and cephaloridine on the indices of cellular and humoral immunity was studied comparatively on intact animals and on animals with secondary immune deficiency .
	manualset3
147895	4	409719	5	NULL	NULL	0	NULL	kanamycin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of ristomycin , chloramphenicol , kanamycin , benzylpenicillin , streptomycin , and cephaloridine on the indices of cellular and humoral immunity was studied comparatively on intact animals and on animals with secondary immune deficiency .
	manualset3
147896	5	409719	5	NULL	NULL	0	NULL	benzylpenicillin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of ristomycin , chloramphenicol , kanamycin , benzylpenicillin , streptomycin , and cephaloridine on the indices of cellular and humoral immunity was studied comparatively on intact animals and on animals with secondary immune deficiency .
	manualset3
147897	6	409719	5	NULL	NULL	0	NULL	streptomycin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of ristomycin , chloramphenicol , kanamycin , benzylpenicillin , streptomycin , and cephaloridine on the indices of cellular and humoral immunity was studied comparatively on intact animals and on animals with secondary immune deficiency .
	manualset3
147898	7	409719	5	NULL	NULL	0	NULL	cephaloridine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of ristomycin , chloramphenicol , kanamycin , benzylpenicillin , streptomycin , and cephaloridine on the indices of cellular and humoral immunity was studied comparatively on intact animals and on animals with secondary immune deficiency .
	manualset3
147899	8	409719	5	NULL	NULL	0	NULL	indices 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of ristomycin , chloramphenicol , kanamycin , benzylpenicillin , streptomycin , and cephaloridine on the indices of cellular and humoral immunity was studied comparatively on intact animals and on animals with secondary immune deficiency .
	manualset3
147900	9	409719	5	NULL	NULL	0	NULL	cellular immunity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of ristomycin , chloramphenicol , kanamycin , benzylpenicillin , streptomycin , and cephaloridine on the indices of cellular and humoral immunity was studied comparatively on intact animals and on animals with secondary immune deficiency .
	manualset3
147901	10	409719	5	NULL	NULL	0	NULL	 humoral immunity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of ristomycin , chloramphenicol , kanamycin , benzylpenicillin , streptomycin , and cephaloridine on the indices of cellular and humoral immunity was studied comparatively on intact animals and on animals with secondary immune deficiency .
	manualset3
147902	11	409719	5	NULL	NULL	0	NULL	intact animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of ristomycin , chloramphenicol , kanamycin , benzylpenicillin , streptomycin , and cephaloridine on the indices of cellular and humoral immunity was studied comparatively on intact animals and on animals with secondary immune deficiency .
	manualset3
147903	12	409719	5	NULL	NULL	0	NULL	animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of ristomycin , chloramphenicol , kanamycin , benzylpenicillin , streptomycin , and cephaloridine on the indices of cellular and humoral immunity was studied comparatively on intact animals and on animals with secondary immune deficiency .
	manualset3
147904	13	409719	5	NULL	NULL	0	NULL	secondary immune deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of ristomycin , chloramphenicol , kanamycin , benzylpenicillin , streptomycin , and cephaloridine on the indices of cellular and humoral immunity was studied comparatively on intact animals and on animals with secondary immune deficiency .
	manualset3
147905	1	409720	5	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of several benzodiazepines ( clonazepam , diazepam , Ro 5-4864 , Ro 15-1788 ) and two pineal gland indoleamines ( N-acetylserotonin , melatonin ) on the spontaneous proliferation of mouse spleen lymphocytes was estimated in vitro by the 3 H-thymidine uptake assay .
	manualset3
147906	2	409720	5	NULL	NULL	0	NULL	benzodiazepines 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of several benzodiazepines ( clonazepam , diazepam , Ro 5-4864 , Ro 15-1788 ) and two pineal gland indoleamines ( N-acetylserotonin , melatonin ) on the spontaneous proliferation of mouse spleen lymphocytes was estimated in vitro by the 3 H-thymidine uptake assay .
	manualset3
147907	3	409720	5	NULL	NULL	0	NULL	clonazepam 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of several benzodiazepines ( clonazepam , diazepam , Ro 5-4864 , Ro 15-1788 ) and two pineal gland indoleamines ( N-acetylserotonin , melatonin ) on the spontaneous proliferation of mouse spleen lymphocytes was estimated in vitro by the 3 H-thymidine uptake assay .
	manualset3
147908	4	409720	5	NULL	NULL	0	NULL	diazepam 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of several benzodiazepines ( clonazepam , diazepam , Ro 5-4864 , Ro 15-1788 ) and two pineal gland indoleamines ( N-acetylserotonin , melatonin ) on the spontaneous proliferation of mouse spleen lymphocytes was estimated in vitro by the 3 H-thymidine uptake assay .
	manualset3
147909	5	409720	5	NULL	NULL	0	NULL	Ro 5-4864 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of several benzodiazepines ( clonazepam , diazepam , Ro 5-4864 , Ro 15-1788 ) and two pineal gland indoleamines ( N-acetylserotonin , melatonin ) on the spontaneous proliferation of mouse spleen lymphocytes was estimated in vitro by the 3 H-thymidine uptake assay .
	manualset3
147910	6	409720	5	NULL	NULL	0	NULL	Ro 15-1788	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of several benzodiazepines ( clonazepam , diazepam , Ro 5-4864 , Ro 15-1788 ) and two pineal gland indoleamines ( N-acetylserotonin , melatonin ) on the spontaneous proliferation of mouse spleen lymphocytes was estimated in vitro by the 3 H-thymidine uptake assay .
	manualset3
147911	7	409720	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of several benzodiazepines ( clonazepam , diazepam , Ro 5-4864 , Ro 15-1788 ) and two pineal gland indoleamines ( N-acetylserotonin , melatonin ) on the spontaneous proliferation of mouse spleen lymphocytes was estimated in vitro by the 3 H-thymidine uptake assay .
	manualset3
147912	8	409720	5	NULL	NULL	0	NULL	pineal gland indoleamines	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of several benzodiazepines ( clonazepam , diazepam , Ro 5-4864 , Ro 15-1788 ) and two pineal gland indoleamines ( N-acetylserotonin , melatonin ) on the spontaneous proliferation of mouse spleen lymphocytes was estimated in vitro by the 3 H-thymidine uptake assay .
	manualset3
147913	9	409720	5	NULL	NULL	0	NULL	N-acetylserotonin	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of several benzodiazepines ( clonazepam , diazepam , Ro 5-4864 , Ro 15-1788 ) and two pineal gland indoleamines ( N-acetylserotonin , melatonin ) on the spontaneous proliferation of mouse spleen lymphocytes was estimated in vitro by the 3 H-thymidine uptake assay .
	manualset3
147914	10	409720	5	NULL	NULL	0	NULL	melatonin 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of several benzodiazepines ( clonazepam , diazepam , Ro 5-4864 , Ro 15-1788 ) and two pineal gland indoleamines ( N-acetylserotonin , melatonin ) on the spontaneous proliferation of mouse spleen lymphocytes was estimated in vitro by the 3 H-thymidine uptake assay .
	manualset3
147915	11	409720	5	NULL	NULL	0	NULL	spontaneous proliferation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of several benzodiazepines ( clonazepam , diazepam , Ro 5-4864 , Ro 15-1788 ) and two pineal gland indoleamines ( N-acetylserotonin , melatonin ) on the spontaneous proliferation of mouse spleen lymphocytes was estimated in vitro by the 3 H-thymidine uptake assay .
	manualset3
147916	12	409720	5	NULL	NULL	0	NULL	mouse spleen lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of several benzodiazepines ( clonazepam , diazepam , Ro 5-4864 , Ro 15-1788 ) and two pineal gland indoleamines ( N-acetylserotonin , melatonin ) on the spontaneous proliferation of mouse spleen lymphocytes was estimated in vitro by the 3 H-thymidine uptake assay .
	manualset3
147917	13	409720	5	NULL	NULL	0	NULL	3 H-thymidine uptake assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of several benzodiazepines ( clonazepam , diazepam , Ro 5-4864 , Ro 15-1788 ) and two pineal gland indoleamines ( N-acetylserotonin , melatonin ) on the spontaneous proliferation of mouse spleen lymphocytes was estimated in vitro by the 3 H-thymidine uptake assay .
	manualset3
147918	1	409721	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of several nucleic acid binding drugs on the cleavage of d ( GGAATTCC ) and pBR 322 by the Eco RI restriction endonuclease .
	manualset3
147919	2	409721	5	NULL	NULL	0	NULL	nucleic acid binding drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of several nucleic acid binding drugs on the cleavage of d ( GGAATTCC ) and pBR 322 by the Eco RI restriction endonuclease .
	manualset3
147920	3	409721	5	NULL	NULL	0	NULL	 cleavage of d ( GGAATTCC )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of several nucleic acid binding drugs on the cleavage of d ( GGAATTCC ) and pBR 322 by the Eco RI restriction endonuclease .
	manualset3
147921	4	409721	5	NULL	NULL	0	NULL	pBR 322	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of several nucleic acid binding drugs on the cleavage of d ( GGAATTCC ) and pBR 322 by the Eco RI restriction endonuclease .
	manualset3
147922	5	409721	5	NULL	NULL	0	NULL	Eco RI restriction endonuclease	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of several nucleic acid binding drugs on the cleavage of d ( GGAATTCC ) and pBR 322 by the Eco RI restriction endonuclease .
	manualset3
147923	1	409722	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of snail control on the prevalence of Schistosoma japonicum infection in the Philippines .
	manualset3
147924	2	409722	5	NULL	NULL	0	NULL	snail control 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of snail control on the prevalence of Schistosoma japonicum infection in the Philippines .
	manualset3
147925	3	409722	5	NULL	NULL	0	NULL	prevalence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of snail control on the prevalence of Schistosoma japonicum infection in the Philippines .
	manualset3
147926	4	409722	5	NULL	NULL	0	NULL	Schistosoma japonicum infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of snail control on the prevalence of Schistosoma japonicum infection in the Philippines .
	manualset3
147927	5	409722	5	NULL	NULL	0	NULL	Philippines 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of snail control on the prevalence of Schistosoma japonicum infection in the Philippines .
	manualset3
147928	1	409723	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of snake venom LAOs on platelet function is controversial .
	manualset3
147929	2	409723	5	NULL	NULL	NULL	NULL	snake venom LAOs 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The effect of snake venom LAOs on platelet function is controversial .
	manualset3
147930	3	409723	5	NULL	NULL	0	NULL	platelet function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of snake venom LAOs on platelet function is controversial .
	manualset3
147931	1	409724	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of steroids on adipogenesis by D1-BAG , a pluripotent cell cloned from mouse bone marrow and transfected with traceable genes encoding beta-galactosidase and neomycin resistance , was investigated in vitro in culture and in vivo after injection into mice .
	manualset3
147932	2	409724	5	NULL	NULL	0	NULL	steroids 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of steroids on adipogenesis by D1-BAG , a pluripotent cell cloned from mouse bone marrow and transfected with traceable genes encoding beta-galactosidase and neomycin resistance , was investigated in vitro in culture and in vivo after injection into mice .
	manualset3
147933	3	409724	5	NULL	NULL	0	NULL	adipogenesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of steroids on adipogenesis by D1-BAG , a pluripotent cell cloned from mouse bone marrow and transfected with traceable genes encoding beta-galactosidase and neomycin resistance , was investigated in vitro in culture and in vivo after injection into mice .
	manualset3
147934	4	409724	5	NULL	NULL	0	NULL	D1-BAG , a pluripotent cell 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of steroids on adipogenesis by D1-BAG , a pluripotent cell cloned from mouse bone marrow and transfected with traceable genes encoding beta-galactosidase and neomycin resistance , was investigated in vitro in culture and in vivo after injection into mice .
	manualset3
147935	5	409724	5	NULL	NULL	0	NULL	mouse bone marrow 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of steroids on adipogenesis by D1-BAG , a pluripotent cell cloned from mouse bone marrow and transfected with traceable genes encoding beta-galactosidase and neomycin resistance , was investigated in vitro in culture and in vivo after injection into mice .
	manualset3
147936	6	409724	5	NULL	NULL	NULL	NULL	traceable genes encoding beta-galactosidase	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The effect of steroids on adipogenesis by D1-BAG , a pluripotent cell cloned from mouse bone marrow and transfected with traceable genes encoding beta-galactosidase and neomycin resistance , was investigated in vitro in culture and in vivo after injection into mice .
	manualset3
147937	7	409724	5	NULL	NULL	NULL	NULL	traceable genes encoding neomycin resistance	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The effect of steroids on adipogenesis by D1-BAG , a pluripotent cell cloned from mouse bone marrow and transfected with traceable genes encoding beta-galactosidase and neomycin resistance , was investigated in vitro in culture and in vivo after injection into mice .
	manualset3
147938	8	409724	5	NULL	NULL	0	NULL	culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of steroids on adipogenesis by D1-BAG , a pluripotent cell cloned from mouse bone marrow and transfected with traceable genes encoding beta-galactosidase and neomycin resistance , was investigated in vitro in culture and in vivo after injection into mice .
	manualset3
147939	9	409724	5	NULL	NULL	0	NULL	injection 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of steroids on adipogenesis by D1-BAG , a pluripotent cell cloned from mouse bone marrow and transfected with traceable genes encoding beta-galactosidase and neomycin resistance , was investigated in vitro in culture and in vivo after injection into mice .
	manualset3
147940	10	409724	5	NULL	NULL	0	NULL	mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of steroids on adipogenesis by D1-BAG , a pluripotent cell cloned from mouse bone marrow and transfected with traceable genes encoding beta-galactosidase and neomycin resistance , was investigated in vitro in culture and in vivo after injection into mice .
	manualset3
147941	1	409725	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of sulfate infusion on calcium excretion .
	manualset3
147942	2	409725	5	NULL	NULL	NULL	NULL	sulfate infusion 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The effect of sulfate infusion on calcium excretion .
	manualset3
147943	3	409725	5	NULL	NULL	0	NULL	calcium excretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of sulfate infusion on calcium excretion .
	manualset3
147944	1	409726	5	NULL	NULL	0	NULL	standard site	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A standard site in the distal shaft of the radius is commonly used to monitor the skeletal status of aging individuals by photon absorptiometry .
	manualset3
147945	2	409726	5	NULL	NULL	0	NULL	distal shaft of the radius	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A standard site in the distal shaft of the radius is commonly used to monitor the skeletal status of aging individuals by photon absorptiometry .
	manualset3
147946	3	409726	5	NULL	NULL	0	NULL	skeletal status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A standard site in the distal shaft of the radius is commonly used to monitor the skeletal status of aging individuals by photon absorptiometry .
	manualset3
147947	4	409726	5	NULL	NULL	0	NULL	aging individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A standard site in the distal shaft of the radius is commonly used to monitor the skeletal status of aging individuals by photon absorptiometry .
	manualset3
147948	5	409726	5	NULL	NULL	0	NULL	photon absorptiometry	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A standard site in the distal shaft of the radius is commonly used to monitor the skeletal status of aging individuals by photon absorptiometry .
	manualset3
147949	1	409727	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the PreS1 fragment of HBV antigen on some neutrophil functions in vitro was also examined .
	manualset3
147950	2	409727	5	NULL	NULL	0	NULL	PreS1 fragment 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the PreS1 fragment of HBV antigen on some neutrophil functions in vitro was also examined .
	manualset3
147951	3	409727	5	NULL	NULL	NULL	NULL	HBV antigen	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The effect of the PreS1 fragment of HBV antigen on some neutrophil functions in vitro was also examined .
	manualset3
147952	4	409727	5	NULL	NULL	0	NULL	neutrophil functions 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the PreS1 fragment of HBV antigen on some neutrophil functions in vitro was also examined .
	manualset3
147953	1	409728	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the dentate lesions appeared to be specific to the behavioral stress : dentate lesions failed to alter resting levels , or the animal 's adrenal responses to laparotomy stress and ether inhalation .
	manualset3
147954	2	409728	5	NULL	NULL	0	NULL	dentate lesions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the dentate lesions appeared to be specific to the behavioral stress : dentate lesions failed to alter resting levels , or the animal 's adrenal responses to laparotomy stress and ether inhalation .
	manualset3
147955	3	409728	5	NULL	NULL	0	NULL	behavioral stress	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the dentate lesions appeared to be specific to the behavioral stress : dentate lesions failed to alter resting levels , or the animal 's adrenal responses to laparotomy stress and ether inhalation .
	manualset3
147956	4	409728	5	NULL	NULL	0	NULL	dentate lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the dentate lesions appeared to be specific to the behavioral stress : dentate lesions failed to alter resting levels , or the animal 's adrenal responses to laparotomy stress and ether inhalation .
	manualset3
147957	5	409728	5	NULL	NULL	0	NULL	resting levels	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the dentate lesions appeared to be specific to the behavioral stress : dentate lesions failed to alter resting levels , or the animal 's adrenal responses to laparotomy stress and ether inhalation .
	manualset3
147958	6	409728	5	NULL	NULL	0	NULL	animal 's adrenal responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the dentate lesions appeared to be specific to the behavioral stress : dentate lesions failed to alter resting levels , or the animal 's adrenal responses to laparotomy stress and ether inhalation .
	manualset3
147959	7	409728	5	NULL	NULL	0	NULL	laparotomy stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the dentate lesions appeared to be specific to the behavioral stress : dentate lesions failed to alter resting levels , or the animal 's adrenal responses to laparotomy stress and ether inhalation .
	manualset3
147960	8	409728	5	NULL	NULL	0	NULL	ether inhalation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the dentate lesions appeared to be specific to the behavioral stress : dentate lesions failed to alter resting levels , or the animal 's adrenal responses to laparotomy stress and ether inhalation .
	manualset3
147961	1	409729	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the haptens 2 , 4-dinitrochlorobenzene ( DNCB ) and 2 , 4-dinitrofluorobenzene ( DNFB ) and of hapten-protein conjugates on the migration of guinea-pig peritoneal exudate cells .
	manualset3
147962	2	409729	5	NULL	NULL	0	NULL	hapten 2 , 4-dinitrochlorobenzene ( DNCB ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the haptens 2 , 4-dinitrochlorobenzene ( DNCB ) and 2 , 4-dinitrofluorobenzene ( DNFB ) and of hapten-protein conjugates on the migration of guinea-pig peritoneal exudate cells .
	manualset3
147963	3	409729	5	NULL	NULL	0	NULL	hapten 2 , 4-dinitrofluorobenzene ( DNFB )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the haptens 2 , 4-dinitrochlorobenzene ( DNCB ) and 2 , 4-dinitrofluorobenzene ( DNFB ) and of hapten-protein conjugates on the migration of guinea-pig peritoneal exudate cells .
	manualset3
147964	4	409729	5	NULL	NULL	0	NULL	hapten-protein conjugates	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the haptens 2 , 4-dinitrochlorobenzene ( DNCB ) and 2 , 4-dinitrofluorobenzene ( DNFB ) and of hapten-protein conjugates on the migration of guinea-pig peritoneal exudate cells .
	manualset3
147970	5	409729	5	NULL	NULL	0	NULL	migration 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the haptens 2 , 4-dinitrochlorobenzene ( DNCB ) and 2 , 4-dinitrofluorobenzene ( DNFB ) and of hapten-protein conjugates on the migration of guinea-pig peritoneal exudate cells .
	manualset3
147971	6	409729	5	NULL	NULL	0	NULL	guinea-pig peritoneal exudate cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the haptens 2 , 4-dinitrochlorobenzene ( DNCB ) and 2 , 4-dinitrofluorobenzene ( DNFB ) and of hapten-protein conjugates on the migration of guinea-pig peritoneal exudate cells .
	manualset3
147972	1	409730	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the selective ET ( B ) antagonist BQ-788 ( 10 ( -12 ) -10 ( -8 ) mole ) on perfusion flow rate and ( 125 ) I-ET-1 extraction was determined .
	manualset3
147973	2	409730	5	NULL	NULL	0	NULL	selective ET ( B ) antagonist BQ-788 ( 10 ( -12 ) -10 ( -8 ) mole ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the selective ET ( B ) antagonist BQ-788 ( 10 ( -12 ) -10 ( -8 ) mole ) on perfusion flow rate and ( 125 ) I-ET-1 extraction was determined .
	manualset3
147974	3	409730	5	NULL	NULL	0	NULL	perfusion flow rate 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the selective ET ( B ) antagonist BQ-788 ( 10 ( -12 ) -10 ( -8 ) mole ) on perfusion flow rate and ( 125 ) I-ET-1 extraction was determined .
	manualset3
147975	4	409730	5	NULL	NULL	0	NULL	( 125 ) I-ET-1 extraction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the selective ET ( B ) antagonist BQ-788 ( 10 ( -12 ) -10 ( -8 ) mole ) on perfusion flow rate and ( 125 ) I-ET-1 extraction was determined .
	manualset3
147976	1	409731	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the washed p ( HEMA ) - Hex-MTX carrier on the morphological structure of donor blood , on blood coagulation indicators and on responses of the living tissue surrounding the material which has been in the blood vessel of the rabbit for various periods of time was evaluated .
	manualset3
147977	2	409731	5	NULL	NULL	0	NULL	washed p ( HEMA ) - Hex-MTX carrier	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the washed p ( HEMA ) - Hex-MTX carrier on the morphological structure of donor blood , on blood coagulation indicators and on responses of the living tissue surrounding the material which has been in the blood vessel of the rabbit for various periods of time was evaluated .
	manualset3
147978	3	409731	5	NULL	NULL	0	NULL	morphological structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the washed p ( HEMA ) - Hex-MTX carrier on the morphological structure of donor blood , on blood coagulation indicators and on responses of the living tissue surrounding the material which has been in the blood vessel of the rabbit for various periods of time was evaluated .
	manualset3
147979	4	409731	5	NULL	NULL	0	NULL	donor blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the washed p ( HEMA ) - Hex-MTX carrier on the morphological structure of donor blood , on blood coagulation indicators and on responses of the living tissue surrounding the material which has been in the blood vessel of the rabbit for various periods of time was evaluated .
	manualset3
147980	5	409731	5	NULL	NULL	0	NULL	blood coagulation indicators	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the washed p ( HEMA ) - Hex-MTX carrier on the morphological structure of donor blood , on blood coagulation indicators and on responses of the living tissue surrounding the material which has been in the blood vessel of the rabbit for various periods of time was evaluated .
	manualset3
147981	6	409731	5	NULL	NULL	0	NULL	responses 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the washed p ( HEMA ) - Hex-MTX carrier on the morphological structure of donor blood , on blood coagulation indicators and on responses of the living tissue surrounding the material which has been in the blood vessel of the rabbit for various periods of time was evaluated .
	manualset3
147982	7	409731	5	NULL	NULL	0	NULL	living tissue 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the washed p ( HEMA ) - Hex-MTX carrier on the morphological structure of donor blood , on blood coagulation indicators and on responses of the living tissue surrounding the material which has been in the blood vessel of the rabbit for various periods of time was evaluated .
	manualset3
147983	8	409731	5	NULL	NULL	0	NULL	material 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the washed p ( HEMA ) - Hex-MTX carrier on the morphological structure of donor blood , on blood coagulation indicators and on responses of the living tissue surrounding the material which has been in the blood vessel of the rabbit for various periods of time was evaluated .
	manualset3
147984	9	409731	5	NULL	NULL	0	NULL	blood vessel 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the washed p ( HEMA ) - Hex-MTX carrier on the morphological structure of donor blood , on blood coagulation indicators and on responses of the living tissue surrounding the material which has been in the blood vessel of the rabbit for various periods of time was evaluated .
	manualset3
147985	10	409731	5	NULL	NULL	0	NULL	rabbit 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the washed p ( HEMA ) - Hex-MTX carrier on the morphological structure of donor blood , on blood coagulation indicators and on responses of the living tissue surrounding the material which has been in the blood vessel of the rabbit for various periods of time was evaluated .
	manualset3
147986	11	409731	5	NULL	NULL	0	NULL	various periods of time	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the washed p ( HEMA ) - Hex-MTX carrier on the morphological structure of donor blood , on blood coagulation indicators and on responses of the living tissue surrounding the material which has been in the blood vessel of the rabbit for various periods of time was evaluated .
	manualset3
147987	1	409732	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the water content in silica glass is greater than the fictive temperature effect and gives larger changes in the amplitude of the elastic modulus for the same thermal dependence .
	manualset3
147988	2	409732	5	NULL	NULL	0	NULL	water content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the water content in silica glass is greater than the fictive temperature effect and gives larger changes in the amplitude of the elastic modulus for the same thermal dependence .
	manualset3
147989	3	409732	5	NULL	NULL	0	NULL	silica glass	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the water content in silica glass is greater than the fictive temperature effect and gives larger changes in the amplitude of the elastic modulus for the same thermal dependence .
	manualset3
147990	4	409732	5	NULL	NULL	0	NULL	fictive temperature effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the water content in silica glass is greater than the fictive temperature effect and gives larger changes in the amplitude of the elastic modulus for the same thermal dependence .
	manualset3
147991	5	409732	5	NULL	NULL	0	NULL	changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the water content in silica glass is greater than the fictive temperature effect and gives larger changes in the amplitude of the elastic modulus for the same thermal dependence .
	manualset3
147992	6	409732	5	NULL	NULL	0	NULL	amplitude 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the water content in silica glass is greater than the fictive temperature effect and gives larger changes in the amplitude of the elastic modulus for the same thermal dependence .
	manualset3
147993	7	409732	5	NULL	NULL	0	NULL	elastic modulus	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the water content in silica glass is greater than the fictive temperature effect and gives larger changes in the amplitude of the elastic modulus for the same thermal dependence .
	manualset3
147994	8	409732	5	NULL	NULL	0	NULL	thermal dependence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of the water content in silica glass is greater than the fictive temperature effect and gives larger changes in the amplitude of the elastic modulus for the same thermal dependence .
	manualset3
147995	1	409733	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of these mutations on the catalytic cycle and the cell biology of the Menkes protein , as well as predictions of the effect of particular mutant MNKs on observed Menkes disease symptoms will also be discussed .
	manualset3
147996	2	409733	5	NULL	NULL	0	NULL	mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of these mutations on the catalytic cycle and the cell biology of the Menkes protein , as well as predictions of the effect of particular mutant MNKs on observed Menkes disease symptoms will also be discussed .
	manualset3
147997	3	409733	5	NULL	NULL	0	NULL	catalytic cycle	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of these mutations on the catalytic cycle and the cell biology of the Menkes protein , as well as predictions of the effect of particular mutant MNKs on observed Menkes disease symptoms will also be discussed .
	manualset3
147998	4	409733	5	NULL	NULL	0	NULL	cell biology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of these mutations on the catalytic cycle and the cell biology of the Menkes protein , as well as predictions of the effect of particular mutant MNKs on observed Menkes disease symptoms will also be discussed .
	manualset3
147999	5	409733	5	NULL	NULL	0	NULL	Menkes protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of these mutations on the catalytic cycle and the cell biology of the Menkes protein , as well as predictions of the effect of particular mutant MNKs on observed Menkes disease symptoms will also be discussed .
	manualset3
148000	6	409733	5	NULL	NULL	0	NULL	predictions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of these mutations on the catalytic cycle and the cell biology of the Menkes protein , as well as predictions of the effect of particular mutant MNKs on observed Menkes disease symptoms will also be discussed .
	manualset3
148001	7	409733	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of these mutations on the catalytic cycle and the cell biology of the Menkes protein , as well as predictions of the effect of particular mutant MNKs on observed Menkes disease symptoms will also be discussed .
	manualset3
148002	8	409733	5	NULL	NULL	0	NULL	particular mutant MNKs	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of these mutations on the catalytic cycle and the cell biology of the Menkes protein , as well as predictions of the effect of particular mutant MNKs on observed Menkes disease symptoms will also be discussed .
	manualset3
148003	9	409733	5	NULL	NULL	0	NULL	Menkes disease symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of these mutations on the catalytic cycle and the cell biology of the Menkes protein , as well as predictions of the effect of particular mutant MNKs on observed Menkes disease symptoms will also be discussed .
	manualset3
148004	1	409734	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of topical treatment with butylated hydroxytoluene ( BHT ) was evaluated in primary and recurrent genital herpes simplex virus type 2 ( HSV-2 ) infection of guinea pigs .
	manualset3
148005	2	409734	5	NULL	NULL	0	NULL	topical treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of topical treatment with butylated hydroxytoluene ( BHT ) was evaluated in primary and recurrent genital herpes simplex virus type 2 ( HSV-2 ) infection of guinea pigs .
	manualset3
148006	3	409734	5	NULL	NULL	0	NULL	butylated hydroxytoluene ( BHT )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of topical treatment with butylated hydroxytoluene ( BHT ) was evaluated in primary and recurrent genital herpes simplex virus type 2 ( HSV-2 ) infection of guinea pigs .
	manualset3
148007	4	409734	5	NULL	NULL	0	NULL	primary genital herpes simplex virus type 2 ( HSV-2 ) infection	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of topical treatment with butylated hydroxytoluene ( BHT ) was evaluated in primary and recurrent genital herpes simplex virus type 2 ( HSV-2 ) infection of guinea pigs .
	manualset3
148008	5	409734	5	NULL	NULL	0	NULL	recurrent genital herpes simplex virus type 2 ( HSV-2 ) infection	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of topical treatment with butylated hydroxytoluene ( BHT ) was evaluated in primary and recurrent genital herpes simplex virus type 2 ( HSV-2 ) infection of guinea pigs .
	manualset3
148009	6	409734	5	NULL	NULL	0	NULL	guinea pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of topical treatment with butylated hydroxytoluene ( BHT ) was evaluated in primary and recurrent genital herpes simplex virus type 2 ( HSV-2 ) infection of guinea pigs .
	manualset3
148010	1	409735	5	NULL	NULL	0	NULL	statistical difference 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A statistical difference was seen between men over 50 years of age compared with younger men , but only for the HOS scores and velocity .
	manualset3
148011	2	409735	5	NULL	NULL	0	NULL	men 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A statistical difference was seen between men over 50 years of age compared with younger men , but only for the HOS scores and velocity .
	manualset3
148012	3	409735	5	NULL	NULL	0	NULL	50 years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A statistical difference was seen between men over 50 years of age compared with younger men , but only for the HOS scores and velocity .
	manualset3
148013	4	409735	5	NULL	NULL	0	NULL	age 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	A statistical difference was seen between men over 50 years of age compared with younger men , but only for the HOS scores and velocity .
	manualset3
148014	5	409735	5	NULL	NULL	0	NULL	younger men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A statistical difference was seen between men over 50 years of age compared with younger men , but only for the HOS scores and velocity .
	manualset3
148015	6	409735	5	NULL	NULL	0	NULL	HOS scores	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A statistical difference was seen between men over 50 years of age compared with younger men , but only for the HOS scores and velocity .
	manualset3
148016	7	409735	5	NULL	NULL	0	NULL	velocity 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A statistical difference was seen between men over 50 years of age compared with younger men , but only for the HOS scores and velocity .
	manualset3
148017	1	409736	5	NULL	NULL	0	NULL	v	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of vigorous exercise during pregnancy .
	manualset3
148018	2	409736	5	NULL	NULL	0	NULL	vigorous exercise 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of vigorous exercise during pregnancy .
	manualset3
148019	3	409736	5	NULL	NULL	0	NULL	pregnancy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of vigorous exercise during pregnancy .
	manualset3
148020	1	409737	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of weight reducing treatments ) .
	manualset3
148021	2	409737	5	NULL	NULL	0	NULL	weight reducing treatments 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of weight reducing treatments ) .
	manualset3
148022	1	409738	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect was also observed when iron was added at the end of the incubation period in the absence of continuing protein synthesis .
	manualset3
148023	2	409738	5	NULL	NULL	0	NULL	iron 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect was also observed when iron was added at the end of the incubation period in the absence of continuing protein synthesis .
	manualset3
148024	3	409738	5	NULL	NULL	0	NULL	incubation period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect was also observed when iron was added at the end of the incubation period in the absence of continuing protein synthesis .
	manualset3
148025	4	409738	5	NULL	NULL	0	NULL	absence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect was also observed when iron was added at the end of the incubation period in the absence of continuing protein synthesis .
	manualset3
148026	5	409738	5	NULL	NULL	0	NULL	protein synthesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect was also observed when iron was added at the end of the incubation period in the absence of continuing protein synthesis .
	manualset3
148027	1	409739	5	NULL	NULL	0	NULL	effective anti-invasive concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effective anti-invasive concentration was 6 micrograms/ml in the pretreatment experiment while 3 micrograms/ml was sufficient to inhibit invasion in the reversibility experiment .
	manualset3
148028	2	409739	5	NULL	NULL	0	NULL	6 micrograms/ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effective anti-invasive concentration was 6 micrograms/ml in the pretreatment experiment while 3 micrograms/ml was sufficient to inhibit invasion in the reversibility experiment .
	manualset3
148029	3	409739	5	NULL	NULL	0	NULL	pretreatment experiment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effective anti-invasive concentration was 6 micrograms/ml in the pretreatment experiment while 3 micrograms/ml was sufficient to inhibit invasion in the reversibility experiment .
	manualset3
148030	4	409739	5	NULL	NULL	NULL	NULL	3 micrograms/ml 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The effective anti-invasive concentration was 6 micrograms/ml in the pretreatment experiment while 3 micrograms/ml was sufficient to inhibit invasion in the reversibility experiment .
	manualset3
148031	5	409739	5	NULL	NULL	0	NULL	invasion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effective anti-invasive concentration was 6 micrograms/ml in the pretreatment experiment while 3 micrograms/ml was sufficient to inhibit invasion in the reversibility experiment .
	manualset3
148032	6	409739	5	NULL	NULL	0	NULL	reversibility experiment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effective anti-invasive concentration was 6 micrograms/ml in the pretreatment experiment while 3 micrograms/ml was sufficient to inhibit invasion in the reversibility experiment .
	manualset3
148033	1	409740	5	NULL	NULL	NULL	NULL	effectiveness 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The effectiveness and mechanism of manganese dioxide ( MnO2 ) enhancing permanganate ( KMnO4 ) oxidation of phenolic compounds were investigated .
	manualset3
148034	2	409740	5	NULL	NULL	0	NULL	mechanism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness and mechanism of manganese dioxide ( MnO2 ) enhancing permanganate ( KMnO4 ) oxidation of phenolic compounds were investigated .
	manualset3
148035	3	409740	5	NULL	NULL	0	NULL	manganese dioxide ( MnO2 ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness and mechanism of manganese dioxide ( MnO2 ) enhancing permanganate ( KMnO4 ) oxidation of phenolic compounds were investigated .
	manualset3
148036	4	409740	5	NULL	NULL	0	NULL	permanganate ( KMnO4 ) oxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness and mechanism of manganese dioxide ( MnO2 ) enhancing permanganate ( KMnO4 ) oxidation of phenolic compounds were investigated .
	manualset3
148037	5	409740	5	NULL	NULL	0	NULL	phenolic compounds	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness and mechanism of manganese dioxide ( MnO2 ) enhancing permanganate ( KMnO4 ) oxidation of phenolic compounds were investigated .
	manualset3
148038	1	409741	5	NULL	NULL	0	NULL	effectiveness 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness of a prandial insulin supplement may have been further improved by a combined basal and meal-related treatment program .
	manualset3
148039	2	409741	5	NULL	NULL	0	NULL	prandial insulin supplement 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness of a prandial insulin supplement may have been further improved by a combined basal and meal-related treatment program .
	manualset3
148040	3	409741	5	NULL	NULL	0	NULL	combined basal and meal-related treatment program	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness of a prandial insulin supplement may have been further improved by a combined basal and meal-related treatment program .
	manualset3
148041	1	409742	5	NULL	NULL	0	NULL	effectiveness 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness of an acetone extraction used to remove extrusion waxes from Pellethane 2363-80A was similarly studied .
	manualset3
148042	2	409742	5	NULL	NULL	0	NULL	acetone extraction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness of an acetone extraction used to remove extrusion waxes from Pellethane 2363-80A was similarly studied .
	manualset3
148043	3	409742	5	NULL	NULL	0	NULL	extrusion waxes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness of an acetone extraction used to remove extrusion waxes from Pellethane 2363-80A was similarly studied .
	manualset3
148044	4	409742	5	NULL	NULL	0	NULL	Pellethane 2363-80A	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness of an acetone extraction used to remove extrusion waxes from Pellethane 2363-80A was similarly studied .
	manualset3
148045	1	409743	5	NULL	NULL	0	NULL	statistical model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A statistical model for mapping specific quantitative trait loci ( QTLs ) that are responsible for allometric scaling laws has been developed .
	manualset3
148046	2	409743	5	NULL	NULL	0	NULL	quantitative trait loci ( QTLs )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A statistical model for mapping specific quantitative trait loci ( QTLs ) that are responsible for allometric scaling laws has been developed .
	manualset3
148047	3	409743	5	NULL	NULL	0	NULL	allometric scaling laws	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A statistical model for mapping specific quantitative trait loci ( QTLs ) that are responsible for allometric scaling laws has been developed .
	manualset3
148048	1	409744	5	NULL	NULL	0	NULL	effectiveness 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness of lindane shampoo ( 1 % gamma benzene hexachloride solution ) was evaluated after one or two time applications to all the children infested .
	manualset3
148049	2	409744	5	NULL	NULL	NULL	NULL	 lindane shampoo ( 1 % gamma benzene hexachloride solution )	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The effectiveness of lindane shampoo ( 1 % gamma benzene hexachloride solution ) was evaluated after one or two time applications to all the children infested .
	manualset3
148050	3	409744	5	NULL	NULL	0	NULL	one or two time applications	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness of lindane shampoo ( 1 % gamma benzene hexachloride solution ) was evaluated after one or two time applications to all the children infested .
	manualset3
148051	4	409744	5	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness of lindane shampoo ( 1 % gamma benzene hexachloride solution ) was evaluated after one or two time applications to all the children infested .
	manualset3
148052	1	409745	5	NULL	NULL	0	NULL	effectiveness 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness of routine outpatient follow up in detecting recurrent disease after ` curative ' surgery for breast cancer has been evaluated in a retrospective study of 148 patients .
	manualset3
148053	2	409745	5	NULL	NULL	0	NULL	routine outpatient follow up 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness of routine outpatient follow up in detecting recurrent disease after ` curative ' surgery for breast cancer has been evaluated in a retrospective study of 148 patients .
	manualset3
148054	3	409745	5	NULL	NULL	0	NULL	recurrent disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness of routine outpatient follow up in detecting recurrent disease after ` curative ' surgery for breast cancer has been evaluated in a retrospective study of 148 patients .
	manualset3
148055	4	409745	5	NULL	NULL	0	NULL	` curative ' surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness of routine outpatient follow up in detecting recurrent disease after ` curative ' surgery for breast cancer has been evaluated in a retrospective study of 148 patients .
	manualset3
148056	5	409745	5	NULL	NULL	0	NULL	breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness of routine outpatient follow up in detecting recurrent disease after ` curative ' surgery for breast cancer has been evaluated in a retrospective study of 148 patients .
	manualset3
148057	6	409745	5	NULL	NULL	0	NULL	retrospective study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness of routine outpatient follow up in detecting recurrent disease after ` curative ' surgery for breast cancer has been evaluated in a retrospective study of 148 patients .
	manualset3
148058	7	409745	5	NULL	NULL	0	NULL	148 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness of routine outpatient follow up in detecting recurrent disease after ` curative ' surgery for breast cancer has been evaluated in a retrospective study of 148 patients .
	manualset3
148059	1	409746	5	NULL	NULL	0	NULL	effectiveness 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness of the approach was assessed with four model compounds , amodiaquine , clozapine , diclofenac , and fipexide , all well-known to form GSH-trapped reactive metabolites , following incubation in human liver microsomes supplemented with - nicotinamide adenine dinucleotide 2 ' - phosphate reduced tetrasodium salt ( NADPH ) and GSH .
	manualset3
148060	2	409746	5	NULL	NULL	0	NULL	approach 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness of the approach was assessed with four model compounds , amodiaquine , clozapine , diclofenac , and fipexide , all well-known to form GSH-trapped reactive metabolites , following incubation in human liver microsomes supplemented with - nicotinamide adenine dinucleotide 2 ' - phosphate reduced tetrasodium salt ( NADPH ) and GSH .
	manualset3
148061	3	409746	5	NULL	NULL	0	NULL	four 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness of the approach was assessed with four model compounds , amodiaquine , clozapine , diclofenac , and fipexide , all well-known to form GSH-trapped reactive metabolites , following incubation in human liver microsomes supplemented with - nicotinamide adenine dinucleotide 2 ' - phosphate reduced tetrasodium salt ( NADPH ) and GSH .
	manualset3
148062	4	409746	5	NULL	NULL	0	NULL	model compound amodiaquine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness of the approach was assessed with four model compounds , amodiaquine , clozapine , diclofenac , and fipexide , all well-known to form GSH-trapped reactive metabolites , following incubation in human liver microsomes supplemented with - nicotinamide adenine dinucleotide 2 ' - phosphate reduced tetrasodium salt ( NADPH ) and GSH .
	manualset3
148063	5	409746	5	NULL	NULL	0	NULL	model compound clozapine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness of the approach was assessed with four model compounds , amodiaquine , clozapine , diclofenac , and fipexide , all well-known to form GSH-trapped reactive metabolites , following incubation in human liver microsomes supplemented with - nicotinamide adenine dinucleotide 2 ' - phosphate reduced tetrasodium salt ( NADPH ) and GSH .
	manualset3
148064	6	409746	5	NULL	NULL	0	NULL	model compound diclofenac 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness of the approach was assessed with four model compounds , amodiaquine , clozapine , diclofenac , and fipexide , all well-known to form GSH-trapped reactive metabolites , following incubation in human liver microsomes supplemented with - nicotinamide adenine dinucleotide 2 ' - phosphate reduced tetrasodium salt ( NADPH ) and GSH .
	manualset3
148065	7	409746	5	NULL	NULL	0	NULL	model compound fipexide 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness of the approach was assessed with four model compounds , amodiaquine , clozapine , diclofenac , and fipexide , all well-known to form GSH-trapped reactive metabolites , following incubation in human liver microsomes supplemented with - nicotinamide adenine dinucleotide 2 ' - phosphate reduced tetrasodium salt ( NADPH ) and GSH .
	manualset3
148066	8	409746	5	NULL	NULL	0	NULL	GSH-trapped reactive metabolites	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness of the approach was assessed with four model compounds , amodiaquine , clozapine , diclofenac , and fipexide , all well-known to form GSH-trapped reactive metabolites , following incubation in human liver microsomes supplemented with - nicotinamide adenine dinucleotide 2 ' - phosphate reduced tetrasodium salt ( NADPH ) and GSH .
	manualset3
148067	9	409746	5	NULL	NULL	0	NULL	incubation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness of the approach was assessed with four model compounds , amodiaquine , clozapine , diclofenac , and fipexide , all well-known to form GSH-trapped reactive metabolites , following incubation in human liver microsomes supplemented with - nicotinamide adenine dinucleotide 2 ' - phosphate reduced tetrasodium salt ( NADPH ) and GSH .
	manualset3
148068	10	409746	5	NULL	NULL	0	NULL	human liver microsomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness of the approach was assessed with four model compounds , amodiaquine , clozapine , diclofenac , and fipexide , all well-known to form GSH-trapped reactive metabolites , following incubation in human liver microsomes supplemented with - nicotinamide adenine dinucleotide 2 ' - phosphate reduced tetrasodium salt ( NADPH ) and GSH .
	manualset3
148069	11	409746	5	NULL	NULL	0	NULL	nicotinamide adenine dinucleotide 2 ' - phosphate reduced tetrasodium salt ( NADPH )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness of the approach was assessed with four model compounds , amodiaquine , clozapine , diclofenac , and fipexide , all well-known to form GSH-trapped reactive metabolites , following incubation in human liver microsomes supplemented with - nicotinamide adenine dinucleotide 2 ' - phosphate reduced tetrasodium salt ( NADPH ) and GSH .
	manualset3
148070	12	409746	5	NULL	NULL	0	NULL	GSH 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effectiveness of the approach was assessed with four model compounds , amodiaquine , clozapine , diclofenac , and fipexide , all well-known to form GSH-trapped reactive metabolites , following incubation in human liver microsomes supplemented with - nicotinamide adenine dinucleotide 2 ' - phosphate reduced tetrasodium salt ( NADPH ) and GSH .
	manualset3
148071	1	409747	5	NULL	NULL	0	NULL	effector cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The effector cells from AML patients poorly responded to interferon stimulation in NK cytolysis .
	manualset3
148072	2	409747	5	NULL	NULL	0	NULL	AML patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The effector cells from AML patients poorly responded to interferon stimulation in NK cytolysis .
	manualset3
148073	3	409747	5	NULL	NULL	0	NULL	interferon stimulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effector cells from AML patients poorly responded to interferon stimulation in NK cytolysis .
	manualset3
148074	4	409747	5	NULL	NULL	0	NULL	NK cytolysis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effector cells from AML patients poorly responded to interferon stimulation in NK cytolysis .
	manualset3
148075	1	409748	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of AMN082 ( 0.1 , 1 or 5mg/kg , intraperitoneally ; 5 or 50nmol , intrathecally ) or diclofenac ( 5mg/kg , intraperitoneally ) administered 30min preprocedure or 3h postprocedure on hindpaw withdrawal latency ( in seconds ) to thermal stimulation , and response threshold ( in grams ) to mechanical stimulation , were measured in adult rats ( n = 6-8 per group ) before and up to 24h after intradermal injection of carrageenan into the hindpaw or hindpaw incision .
	manualset3
148076	2	409748	5	NULL	NULL	0	NULL	AMN082 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of AMN082 ( 0.1 , 1 or 5mg/kg , intraperitoneally ; 5 or 50nmol , intrathecally ) or diclofenac ( 5mg/kg , intraperitoneally ) administered 30min preprocedure or 3h postprocedure on hindpaw withdrawal latency ( in seconds ) to thermal stimulation , and response threshold ( in grams ) to mechanical stimulation , were measured in adult rats ( n = 6-8 per group ) before and up to 24h after intradermal injection of carrageenan into the hindpaw or hindpaw incision .
	manualset3
148077	3	409748	5	NULL	NULL	0	NULL	 0.1 , 1 or 5mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of AMN082 ( 0.1 , 1 or 5mg/kg , intraperitoneally ; 5 or 50nmol , intrathecally ) or diclofenac ( 5mg/kg , intraperitoneally ) administered 30min preprocedure or 3h postprocedure on hindpaw withdrawal latency ( in seconds ) to thermal stimulation , and response threshold ( in grams ) to mechanical stimulation , were measured in adult rats ( n = 6-8 per group ) before and up to 24h after intradermal injection of carrageenan into the hindpaw or hindpaw incision .
	manualset3
148078	4	409748	5	NULL	NULL	0	NULL	5 or 50nmol 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of AMN082 ( 0.1 , 1 or 5mg/kg , intraperitoneally ; 5 or 50nmol , intrathecally ) or diclofenac ( 5mg/kg , intraperitoneally ) administered 30min preprocedure or 3h postprocedure on hindpaw withdrawal latency ( in seconds ) to thermal stimulation , and response threshold ( in grams ) to mechanical stimulation , were measured in adult rats ( n = 6-8 per group ) before and up to 24h after intradermal injection of carrageenan into the hindpaw or hindpaw incision .
	manualset3
148079	5	409748	5	NULL	NULL	0	NULL	diclofenac 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of AMN082 ( 0.1 , 1 or 5mg/kg , intraperitoneally ; 5 or 50nmol , intrathecally ) or diclofenac ( 5mg/kg , intraperitoneally ) administered 30min preprocedure or 3h postprocedure on hindpaw withdrawal latency ( in seconds ) to thermal stimulation , and response threshold ( in grams ) to mechanical stimulation , were measured in adult rats ( n = 6-8 per group ) before and up to 24h after intradermal injection of carrageenan into the hindpaw or hindpaw incision .
	manualset3
148080	6	409748	5	NULL	NULL	0	NULL	5mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of AMN082 ( 0.1 , 1 or 5mg/kg , intraperitoneally ; 5 or 50nmol , intrathecally ) or diclofenac ( 5mg/kg , intraperitoneally ) administered 30min preprocedure or 3h postprocedure on hindpaw withdrawal latency ( in seconds ) to thermal stimulation , and response threshold ( in grams ) to mechanical stimulation , were measured in adult rats ( n = 6-8 per group ) before and up to 24h after intradermal injection of carrageenan into the hindpaw or hindpaw incision .
	manualset3
148081	7	409748	5	NULL	NULL	0	NULL	30min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of AMN082 ( 0.1 , 1 or 5mg/kg , intraperitoneally ; 5 or 50nmol , intrathecally ) or diclofenac ( 5mg/kg , intraperitoneally ) administered 30min preprocedure or 3h postprocedure on hindpaw withdrawal latency ( in seconds ) to thermal stimulation , and response threshold ( in grams ) to mechanical stimulation , were measured in adult rats ( n = 6-8 per group ) before and up to 24h after intradermal injection of carrageenan into the hindpaw or hindpaw incision .
	manualset3
148082	8	409748	5	NULL	NULL	0	NULL	 3h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of AMN082 ( 0.1 , 1 or 5mg/kg , intraperitoneally ; 5 or 50nmol , intrathecally ) or diclofenac ( 5mg/kg , intraperitoneally ) administered 30min preprocedure or 3h postprocedure on hindpaw withdrawal latency ( in seconds ) to thermal stimulation , and response threshold ( in grams ) to mechanical stimulation , were measured in adult rats ( n = 6-8 per group ) before and up to 24h after intradermal injection of carrageenan into the hindpaw or hindpaw incision .
	manualset3
148083	9	409748	5	NULL	NULL	NULL	NULL	hindpaw withdrawal latency 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The effects of AMN082 ( 0.1 , 1 or 5mg/kg , intraperitoneally ; 5 or 50nmol , intrathecally ) or diclofenac ( 5mg/kg , intraperitoneally ) administered 30min preprocedure or 3h postprocedure on hindpaw withdrawal latency ( in seconds ) to thermal stimulation , and response threshold ( in grams ) to mechanical stimulation , were measured in adult rats ( n = 6-8 per group ) before and up to 24h after intradermal injection of carrageenan into the hindpaw or hindpaw incision .
	manualset3
148084	10	409748	5	NULL	NULL	0	NULL	seconds 	Unit												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of AMN082 ( 0.1 , 1 or 5mg/kg , intraperitoneally ; 5 or 50nmol , intrathecally ) or diclofenac ( 5mg/kg , intraperitoneally ) administered 30min preprocedure or 3h postprocedure on hindpaw withdrawal latency ( in seconds ) to thermal stimulation , and response threshold ( in grams ) to mechanical stimulation , were measured in adult rats ( n = 6-8 per group ) before and up to 24h after intradermal injection of carrageenan into the hindpaw or hindpaw incision .
	manualset3
148085	11	409748	5	NULL	NULL	0	NULL	thermal stimulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of AMN082 ( 0.1 , 1 or 5mg/kg , intraperitoneally ; 5 or 50nmol , intrathecally ) or diclofenac ( 5mg/kg , intraperitoneally ) administered 30min preprocedure or 3h postprocedure on hindpaw withdrawal latency ( in seconds ) to thermal stimulation , and response threshold ( in grams ) to mechanical stimulation , were measured in adult rats ( n = 6-8 per group ) before and up to 24h after intradermal injection of carrageenan into the hindpaw or hindpaw incision .
	manualset3
148086	12	409748	5	NULL	NULL	0	NULL	response threshold 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of AMN082 ( 0.1 , 1 or 5mg/kg , intraperitoneally ; 5 or 50nmol , intrathecally ) or diclofenac ( 5mg/kg , intraperitoneally ) administered 30min preprocedure or 3h postprocedure on hindpaw withdrawal latency ( in seconds ) to thermal stimulation , and response threshold ( in grams ) to mechanical stimulation , were measured in adult rats ( n = 6-8 per group ) before and up to 24h after intradermal injection of carrageenan into the hindpaw or hindpaw incision .
	manualset3
148087	13	409748	5	NULL	NULL	0	NULL	grams 	Unit												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of AMN082 ( 0.1 , 1 or 5mg/kg , intraperitoneally ; 5 or 50nmol , intrathecally ) or diclofenac ( 5mg/kg , intraperitoneally ) administered 30min preprocedure or 3h postprocedure on hindpaw withdrawal latency ( in seconds ) to thermal stimulation , and response threshold ( in grams ) to mechanical stimulation , were measured in adult rats ( n = 6-8 per group ) before and up to 24h after intradermal injection of carrageenan into the hindpaw or hindpaw incision .
	manualset3
148088	14	409748	5	NULL	NULL	0	NULL	mechanical stimulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of AMN082 ( 0.1 , 1 or 5mg/kg , intraperitoneally ; 5 or 50nmol , intrathecally ) or diclofenac ( 5mg/kg , intraperitoneally ) administered 30min preprocedure or 3h postprocedure on hindpaw withdrawal latency ( in seconds ) to thermal stimulation , and response threshold ( in grams ) to mechanical stimulation , were measured in adult rats ( n = 6-8 per group ) before and up to 24h after intradermal injection of carrageenan into the hindpaw or hindpaw incision .
	manualset3
148089	15	409748	5	NULL	NULL	0	NULL	adult rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of AMN082 ( 0.1 , 1 or 5mg/kg , intraperitoneally ; 5 or 50nmol , intrathecally ) or diclofenac ( 5mg/kg , intraperitoneally ) administered 30min preprocedure or 3h postprocedure on hindpaw withdrawal latency ( in seconds ) to thermal stimulation , and response threshold ( in grams ) to mechanical stimulation , were measured in adult rats ( n = 6-8 per group ) before and up to 24h after intradermal injection of carrageenan into the hindpaw or hindpaw incision .
	manualset3
148090	16	409748	5	NULL	NULL	0	NULL	n = 6-8 per group 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of AMN082 ( 0.1 , 1 or 5mg/kg , intraperitoneally ; 5 or 50nmol , intrathecally ) or diclofenac ( 5mg/kg , intraperitoneally ) administered 30min preprocedure or 3h postprocedure on hindpaw withdrawal latency ( in seconds ) to thermal stimulation , and response threshold ( in grams ) to mechanical stimulation , were measured in adult rats ( n = 6-8 per group ) before and up to 24h after intradermal injection of carrageenan into the hindpaw or hindpaw incision .
	manualset3
148091	17	409748	5	NULL	NULL	0	NULL	24h 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of AMN082 ( 0.1 , 1 or 5mg/kg , intraperitoneally ; 5 or 50nmol , intrathecally ) or diclofenac ( 5mg/kg , intraperitoneally ) administered 30min preprocedure or 3h postprocedure on hindpaw withdrawal latency ( in seconds ) to thermal stimulation , and response threshold ( in grams ) to mechanical stimulation , were measured in adult rats ( n = 6-8 per group ) before and up to 24h after intradermal injection of carrageenan into the hindpaw or hindpaw incision .
	manualset3
148092	18	409748	5	NULL	NULL	0	NULL	intradermal injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of AMN082 ( 0.1 , 1 or 5mg/kg , intraperitoneally ; 5 or 50nmol , intrathecally ) or diclofenac ( 5mg/kg , intraperitoneally ) administered 30min preprocedure or 3h postprocedure on hindpaw withdrawal latency ( in seconds ) to thermal stimulation , and response threshold ( in grams ) to mechanical stimulation , were measured in adult rats ( n = 6-8 per group ) before and up to 24h after intradermal injection of carrageenan into the hindpaw or hindpaw incision .
	manualset3
148093	19	409748	5	NULL	NULL	0	NULL	carrageenan 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of AMN082 ( 0.1 , 1 or 5mg/kg , intraperitoneally ; 5 or 50nmol , intrathecally ) or diclofenac ( 5mg/kg , intraperitoneally ) administered 30min preprocedure or 3h postprocedure on hindpaw withdrawal latency ( in seconds ) to thermal stimulation , and response threshold ( in grams ) to mechanical stimulation , were measured in adult rats ( n = 6-8 per group ) before and up to 24h after intradermal injection of carrageenan into the hindpaw or hindpaw incision .
	manualset3
148094	20	409748	5	NULL	NULL	0	NULL	hindpaw 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of AMN082 ( 0.1 , 1 or 5mg/kg , intraperitoneally ; 5 or 50nmol , intrathecally ) or diclofenac ( 5mg/kg , intraperitoneally ) administered 30min preprocedure or 3h postprocedure on hindpaw withdrawal latency ( in seconds ) to thermal stimulation , and response threshold ( in grams ) to mechanical stimulation , were measured in adult rats ( n = 6-8 per group ) before and up to 24h after intradermal injection of carrageenan into the hindpaw or hindpaw incision .
	manualset3
148095	21	409748	5	NULL	NULL	0	NULL	hindpaw incision	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of AMN082 ( 0.1 , 1 or 5mg/kg , intraperitoneally ; 5 or 50nmol , intrathecally ) or diclofenac ( 5mg/kg , intraperitoneally ) administered 30min preprocedure or 3h postprocedure on hindpaw withdrawal latency ( in seconds ) to thermal stimulation , and response threshold ( in grams ) to mechanical stimulation , were measured in adult rats ( n = 6-8 per group ) before and up to 24h after intradermal injection of carrageenan into the hindpaw or hindpaw incision .
	manualset3
148096	1	409749	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of BQ123 , a selective ETA receptor antagonist , on ET-1-induced growth were then assessed .
	manualset3
148097	2	409749	5	NULL	NULL	0	NULL	BQ123 , a selective ETA receptor antagonist	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of BQ123 , a selective ETA receptor antagonist , on ET-1-induced growth were then assessed .
	manualset3
148098	3	409749	5	NULL	NULL	0	NULL	ET-1-induced growth	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of BQ123 , a selective ETA receptor antagonist , on ET-1-induced growth were then assessed .
	manualset3
148099	1	409750	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of D-penicillamine on taste preference and volume intake of sodium chloride by the rat .
	manualset3
148100	2	409750	5	NULL	NULL	0	NULL	D-penicillamine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of D-penicillamine on taste preference and volume intake of sodium chloride by the rat .
	manualset3
148101	3	409750	5	NULL	NULL	0	NULL	taste preference 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of D-penicillamine on taste preference and volume intake of sodium chloride by the rat .
	manualset3
148102	4	409750	5	NULL	NULL	0	NULL	volume intake 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of D-penicillamine on taste preference and volume intake of sodium chloride by the rat .
	manualset3
148103	5	409750	5	NULL	NULL	0	NULL	sodium chloride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of D-penicillamine on taste preference and volume intake of sodium chloride by the rat .
	manualset3
148104	6	409750	5	NULL	NULL	0	NULL	rat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of D-penicillamine on taste preference and volume intake of sodium chloride by the rat .
	manualset3
148105	1	409751	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of DAPB and its metabolites on pentobarbital ( PB ) - induced sleep were examined after i.p. , i.v. and i.c.v. administration .
	manualset3
148106	2	409751	5	NULL	NULL	0	NULL	DAPB 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of DAPB and its metabolites on pentobarbital ( PB ) - induced sleep were examined after i.p. , i.v. and i.c.v. administration .
	manualset3
148107	3	409751	5	NULL	NULL	0	NULL	metabolites 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of DAPB and its metabolites on pentobarbital ( PB ) - induced sleep were examined after i.p. , i.v. and i.c.v. administration .
	manualset3
148108	4	409751	5	NULL	NULL	0	NULL	pentobarbital ( PB ) - induced sleep 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of DAPB and its metabolites on pentobarbital ( PB ) - induced sleep were examined after i.p. , i.v. and i.c.v. administration .
	manualset3
148109	5	409751	5	NULL	NULL	0	NULL	 i.p. administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of DAPB and its metabolites on pentobarbital ( PB ) - induced sleep were examined after i.p. , i.v. and i.c.v. administration .
	manualset3
148110	6	409751	5	NULL	NULL	0	NULL	i.v. administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of DAPB and its metabolites on pentobarbital ( PB ) - induced sleep were examined after i.p. , i.v. and i.c.v. administration .
	manualset3
148111	7	409751	5	NULL	NULL	0	NULL	i.c.v. administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of DAPB and its metabolites on pentobarbital ( PB ) - induced sleep were examined after i.p. , i.v. and i.c.v. administration .
	manualset3
148112	1	409752	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of IgA immune complex ( IgA-IC ) on the contractile function of cultured mesangial cells were measured by the changes in planar surface area in response to treatment with agonists .
	manualset3
148113	2	409752	5	NULL	NULL	0	NULL	IgA immune complex ( IgA-IC ) 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of IgA immune complex ( IgA-IC ) on the contractile function of cultured mesangial cells were measured by the changes in planar surface area in response to treatment with agonists .
	manualset3
148114	3	409752	5	NULL	NULL	0	NULL	contractile function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of IgA immune complex ( IgA-IC ) on the contractile function of cultured mesangial cells were measured by the changes in planar surface area in response to treatment with agonists .
	manualset3
148115	4	409752	5	NULL	NULL	0	NULL	cultured mesangial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of IgA immune complex ( IgA-IC ) on the contractile function of cultured mesangial cells were measured by the changes in planar surface area in response to treatment with agonists .
	manualset3
148116	5	409752	5	NULL	NULL	0	NULL	changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of IgA immune complex ( IgA-IC ) on the contractile function of cultured mesangial cells were measured by the changes in planar surface area in response to treatment with agonists .
	manualset3
148117	6	409752	5	NULL	NULL	0	NULL	planar surface area	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of IgA immune complex ( IgA-IC ) on the contractile function of cultured mesangial cells were measured by the changes in planar surface area in response to treatment with agonists .
	manualset3
148118	7	409752	5	NULL	NULL	0	NULL	response 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of IgA immune complex ( IgA-IC ) on the contractile function of cultured mesangial cells were measured by the changes in planar surface area in response to treatment with agonists .
	manualset3
148119	8	409752	5	NULL	NULL	0	NULL	treatment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of IgA immune complex ( IgA-IC ) on the contractile function of cultured mesangial cells were measured by the changes in planar surface area in response to treatment with agonists .
	manualset3
148120	9	409752	5	NULL	NULL	0	NULL	agonists 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of IgA immune complex ( IgA-IC ) on the contractile function of cultured mesangial cells were measured by the changes in planar surface area in response to treatment with agonists .
	manualset3
148121	1	409753	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of NO on these currents are mediated by the activation of guanylyl cyclase ( GC ) , since they are prevented by Methylene Blue , an inhibitor of GC , and by ODQ , a specific inhibitor of the soluble form of GC .
	manualset3
148122	2	409753	5	NULL	NULL	0	NULL	NO 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of NO on these currents are mediated by the activation of guanylyl cyclase ( GC ) , since they are prevented by Methylene Blue , an inhibitor of GC , and by ODQ , a specific inhibitor of the soluble form of GC .
	manualset3
148123	3	409753	5	NULL	NULL	0	NULL	currents 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of NO on these currents are mediated by the activation of guanylyl cyclase ( GC ) , since they are prevented by Methylene Blue , an inhibitor of GC , and by ODQ , a specific inhibitor of the soluble form of GC .
	manualset3
148124	4	409753	5	NULL	NULL	0	NULL	activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of NO on these currents are mediated by the activation of guanylyl cyclase ( GC ) , since they are prevented by Methylene Blue , an inhibitor of GC , and by ODQ , a specific inhibitor of the soluble form of GC .
	manualset3
148125	5	409753	5	NULL	NULL	0	NULL	guanylyl cyclase ( GC )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of NO on these currents are mediated by the activation of guanylyl cyclase ( GC ) , since they are prevented by Methylene Blue , an inhibitor of GC , and by ODQ , a specific inhibitor of the soluble form of GC .
	manualset3
148126	6	409753	5	NULL	NULL	0	NULL	Methylene Blue , an inhibitor of GC	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of NO on these currents are mediated by the activation of guanylyl cyclase ( GC ) , since they are prevented by Methylene Blue , an inhibitor of GC , and by ODQ , a specific inhibitor of the soluble form of GC .
	manualset3
148127	7	409753	5	NULL	NULL	0	NULL	ODQ , a specific inhibitor of the soluble form of GC	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of NO on these currents are mediated by the activation of guanylyl cyclase ( GC ) , since they are prevented by Methylene Blue , an inhibitor of GC , and by ODQ , a specific inhibitor of the soluble form of GC .
	manualset3
148128	1	409754	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of SQ1 and its reversal by 25-hydroxycholesterol and the effects of bile acids were reproduced in reporter gene assays with a phenobarbital-responsive enhancer unit of CYP2H1 .
	manualset3
148129	2	409754	5	NULL	NULL	0	NULL	SQ1 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of SQ1 and its reversal by 25-hydroxycholesterol and the effects of bile acids were reproduced in reporter gene assays with a phenobarbital-responsive enhancer unit of CYP2H1 .
	manualset3
148130	3	409754	5	NULL	NULL	0	NULL	reversal 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of SQ1 and its reversal by 25-hydroxycholesterol and the effects of bile acids were reproduced in reporter gene assays with a phenobarbital-responsive enhancer unit of CYP2H1 .
	manualset3
148131	4	409754	5	NULL	NULL	0	NULL	25-hydroxycholesterol 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of SQ1 and its reversal by 25-hydroxycholesterol and the effects of bile acids were reproduced in reporter gene assays with a phenobarbital-responsive enhancer unit of CYP2H1 .
	manualset3
148132	5	409754	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of SQ1 and its reversal by 25-hydroxycholesterol and the effects of bile acids were reproduced in reporter gene assays with a phenobarbital-responsive enhancer unit of CYP2H1 .
	manualset3
148133	6	409754	5	NULL	NULL	0	NULL	bile acids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of SQ1 and its reversal by 25-hydroxycholesterol and the effects of bile acids were reproduced in reporter gene assays with a phenobarbital-responsive enhancer unit of CYP2H1 .
	manualset3
148134	7	409754	5	NULL	NULL	0	NULL	reporter gene assays 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of SQ1 and its reversal by 25-hydroxycholesterol and the effects of bile acids were reproduced in reporter gene assays with a phenobarbital-responsive enhancer unit of CYP2H1 .
	manualset3
148135	8	409754	5	NULL	NULL	0	NULL	phenobarbital-responsive enhancer unit	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of SQ1 and its reversal by 25-hydroxycholesterol and the effects of bile acids were reproduced in reporter gene assays with a phenobarbital-responsive enhancer unit of CYP2H1 .
	manualset3
148136	9	409754	5	NULL	NULL	0	NULL	CYP2H1 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of SQ1 and its reversal by 25-hydroxycholesterol and the effects of bile acids were reproduced in reporter gene assays with a phenobarbital-responsive enhancer unit of CYP2H1 .
	manualset3
148137	1	409755	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of YopP on the immune response were studied by a Yersinia Ag-independent approach using bacteria that translocate the well-characterized model Ag listeriolysin O of Listeria monocytogenes via their type III secretion system .
	manualset3
148138	2	409755	5	NULL	NULL	0	NULL	YopP 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of YopP on the immune response were studied by a Yersinia Ag-independent approach using bacteria that translocate the well-characterized model Ag listeriolysin O of Listeria monocytogenes via their type III secretion system .
	manualset3
148139	3	409755	5	NULL	NULL	0	NULL	immune response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of YopP on the immune response were studied by a Yersinia Ag-independent approach using bacteria that translocate the well-characterized model Ag listeriolysin O of Listeria monocytogenes via their type III secretion system .
	manualset3
148140	4	409755	5	NULL	NULL	0	NULL	Yersinia Ag-independent approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of YopP on the immune response were studied by a Yersinia Ag-independent approach using bacteria that translocate the well-characterized model Ag listeriolysin O of Listeria monocytogenes via their type III secretion system .
	manualset3
148141	5	409755	5	NULL	NULL	0	NULL	bacteria 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of YopP on the immune response were studied by a Yersinia Ag-independent approach using bacteria that translocate the well-characterized model Ag listeriolysin O of Listeria monocytogenes via their type III secretion system .
	manualset3
148142	6	409755	5	NULL	NULL	0	NULL	well-characterized model Ag listeriolysin O	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of YopP on the immune response were studied by a Yersinia Ag-independent approach using bacteria that translocate the well-characterized model Ag listeriolysin O of Listeria monocytogenes via their type III secretion system .
	manualset3
148143	7	409755	5	NULL	NULL	0	NULL	Listeria monocytogenes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of YopP on the immune response were studied by a Yersinia Ag-independent approach using bacteria that translocate the well-characterized model Ag listeriolysin O of Listeria monocytogenes via their type III secretion system .
	manualset3
148144	8	409755	5	NULL	NULL	0	NULL	type III secretion system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of YopP on the immune response were studied by a Yersinia Ag-independent approach using bacteria that translocate the well-characterized model Ag listeriolysin O of Listeria monocytogenes via their type III secretion system .
	manualset3
148145	1	409756	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of a diet enriched in magnesium were studied in mineralocorticoid DOCA-salt hypertensive rats from 6 to 15 weeks old , during the development of hypertension .
	manualset3
148146	2	409756	5	NULL	NULL	0	NULL	diet enriched in magnesium 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of a diet enriched in magnesium were studied in mineralocorticoid DOCA-salt hypertensive rats from 6 to 15 weeks old , during the development of hypertension .
	manualset3
148147	3	409756	5	NULL	NULL	0	NULL	mineralocorticoid DOCA-salt hypertensive rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of a diet enriched in magnesium were studied in mineralocorticoid DOCA-salt hypertensive rats from 6 to 15 weeks old , during the development of hypertension .
	manualset3
148148	4	409756	5	NULL	NULL	0	NULL	6 to 15 weeks old	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of a diet enriched in magnesium were studied in mineralocorticoid DOCA-salt hypertensive rats from 6 to 15 weeks old , during the development of hypertension .
	manualset3
148149	5	409756	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of a diet enriched in magnesium were studied in mineralocorticoid DOCA-salt hypertensive rats from 6 to 15 weeks old , during the development of hypertension .
	manualset3
148150	6	409756	5	NULL	NULL	0	NULL	hypertension 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of a diet enriched in magnesium were studied in mineralocorticoid DOCA-salt hypertensive rats from 6 to 15 weeks old , during the development of hypertension .
	manualset3
148151	1	409757	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of a new monochrome mast cell stabilizer ( FPL 52694 ) on gastric secretion have been studied in healthy volunteers .
	manualset3
148152	2	409757	5	NULL	NULL	0	NULL	monochrome mast cell stabilizer ( FPL 52694 ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of a new monochrome mast cell stabilizer ( FPL 52694 ) on gastric secretion have been studied in healthy volunteers .
	manualset3
148153	3	409757	5	NULL	NULL	0	NULL	gastric secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of a new monochrome mast cell stabilizer ( FPL 52694 ) on gastric secretion have been studied in healthy volunteers .
	manualset3
148154	4	409757	5	NULL	NULL	0	NULL	healthy volunteers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of a new monochrome mast cell stabilizer ( FPL 52694 ) on gastric secretion have been studied in healthy volunteers .
	manualset3
148155	1	409758	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of age and sex on the expression of estrogen and its receptors in rat mandibular condylar cartilages .
	manualset3
148156	2	409758	5	NULL	NULL	0	NULL	age 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of age and sex on the expression of estrogen and its receptors in rat mandibular condylar cartilages .
	manualset3
148157	3	409758	5	NULL	NULL	0	NULL	sex 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of age and sex on the expression of estrogen and its receptors in rat mandibular condylar cartilages .
	manualset3
148158	4	409758	5	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of age and sex on the expression of estrogen and its receptors in rat mandibular condylar cartilages .
	manualset3
148159	5	409758	5	NULL	NULL	0	NULL	estrogen 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of age and sex on the expression of estrogen and its receptors in rat mandibular condylar cartilages .
	manualset3
148160	6	409758	5	NULL	NULL	0	NULL	estrogen receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of age and sex on the expression of estrogen and its receptors in rat mandibular condylar cartilages .
	manualset3
148161	7	409758	5	NULL	NULL	0	NULL	rat mandibular condylar cartilages	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of age and sex on the expression of estrogen and its receptors in rat mandibular condylar cartilages .
	manualset3
148162	1	409759	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of alginate coated on tetracycline ( Tc ) loaded poly ( D , L-lactic-co-glycolic acid ) ( PLGA ) microspheres fabricated by double emulsion solvent evaporation technique for local delivery to periodontal pocket were investigated .
	manualset3
148163	2	409759	5	NULL	NULL	0	NULL	alginate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of alginate coated on tetracycline ( Tc ) loaded poly ( D , L-lactic-co-glycolic acid ) ( PLGA ) microspheres fabricated by double emulsion solvent evaporation technique for local delivery to periodontal pocket were investigated .
	manualset3
148164	3	409759	5	NULL	NULL	0	NULL	tetracycline ( Tc ) loaded poly ( D , L-lactic-co-glycolic acid ) ( PLGA ) microspheres	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of alginate coated on tetracycline ( Tc ) loaded poly ( D , L-lactic-co-glycolic acid ) ( PLGA ) microspheres fabricated by double emulsion solvent evaporation technique for local delivery to periodontal pocket were investigated .
	manualset3
148165	4	409759	5	NULL	NULL	0	NULL	double emulsion solvent evaporation technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of alginate coated on tetracycline ( Tc ) loaded poly ( D , L-lactic-co-glycolic acid ) ( PLGA ) microspheres fabricated by double emulsion solvent evaporation technique for local delivery to periodontal pocket were investigated .
	manualset3
148167	5	409759	5	NULL	NULL	0	NULL	periodontal pocket	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of alginate coated on tetracycline ( Tc ) loaded poly ( D , L-lactic-co-glycolic acid ) ( PLGA ) microspheres fabricated by double emulsion solvent evaporation technique for local delivery to periodontal pocket were investigated .
	manualset3
148168	1	409760	5	NULL	NULL	0	NULL	significant excess 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A statistically significant excess of lung cancer ( SMR 136 ) was found .
	manualset3
148169	2	409760	5	NULL	NULL	0	NULL	lung cancer ( SMR 136 )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A statistically significant excess of lung cancer ( SMR 136 ) was found .
	manualset3
148170	1	409761	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of antioxidant drugs on retinal ischemia-reperfusion damage were studied by electroretinograms ( ERGs ) from reperfused Dutch rabbit eyes .
	manualset3
148171	2	409761	5	NULL	NULL	0	NULL	antioxidant drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of antioxidant drugs on retinal ischemia-reperfusion damage were studied by electroretinograms ( ERGs ) from reperfused Dutch rabbit eyes .
	manualset3
148172	3	409761	5	NULL	NULL	0	NULL	retinal ischemia-reperfusion damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of antioxidant drugs on retinal ischemia-reperfusion damage were studied by electroretinograms ( ERGs ) from reperfused Dutch rabbit eyes .
	manualset3
148173	4	409761	5	NULL	NULL	0	NULL	electroretinograms ( ERGs )	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of antioxidant drugs on retinal ischemia-reperfusion damage were studied by electroretinograms ( ERGs ) from reperfused Dutch rabbit eyes .
	manualset3
148174	5	409761	5	NULL	NULL	0	NULL	reperfused Dutch rabbit eyes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of antioxidant drugs on retinal ischemia-reperfusion damage were studied by electroretinograms ( ERGs ) from reperfused Dutch rabbit eyes .
	manualset3
148175	1	409762	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of body mass index on changes in prostate-specific antigen levels and prostate volume over 15 years of follow-up : implications for prostate cancer detection .
	manualset3
148176	2	409762	5	NULL	NULL	0	NULL	body mass index 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of body mass index on changes in prostate-specific antigen levels and prostate volume over 15 years of follow-up : implications for prostate cancer detection .
	manualset3
148177	3	409762	5	NULL	NULL	0	NULL	changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of body mass index on changes in prostate-specific antigen levels and prostate volume over 15 years of follow-up : implications for prostate cancer detection .
	manualset3
148178	4	409762	5	NULL	NULL	0	NULL	prostate-specific antigen levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of body mass index on changes in prostate-specific antigen levels and prostate volume over 15 years of follow-up : implications for prostate cancer detection .
	manualset3
148179	5	409762	5	NULL	NULL	0	NULL	prostate volume	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of body mass index on changes in prostate-specific antigen levels and prostate volume over 15 years of follow-up : implications for prostate cancer detection .
	manualset3
148180	6	409762	5	NULL	NULL	0	NULL	15 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of body mass index on changes in prostate-specific antigen levels and prostate volume over 15 years of follow-up : implications for prostate cancer detection .
	manualset3
148181	7	409762	5	NULL	NULL	0	NULL	implications 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of body mass index on changes in prostate-specific antigen levels and prostate volume over 15 years of follow-up : implications for prostate cancer detection .
	manualset3
148182	8	409762	5	NULL	NULL	0	NULL	prostate cancer detection 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of body mass index on changes in prostate-specific antigen levels and prostate volume over 15 years of follow-up : implications for prostate cancer detection .
	manualset3
148183	1	409763	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of cations on labyrinthine activity .
	manualset3
148184	2	409763	5	NULL	NULL	0	NULL	cations 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of cations on labyrinthine activity .
	manualset3
148185	3	409763	5	NULL	NULL	0	NULL	labyrinthine activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of cations on labyrinthine activity .
	manualset3
148186	1	409764	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of chronic elevations of growth hormone levels on hepatic insulin binding and action were studied in rats with subcutaneously implanted growth hormone-producing tumors .
	manualset3
148187	2	409764	5	NULL	NULL	0	NULL	chronic elevations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of chronic elevations of growth hormone levels on hepatic insulin binding and action were studied in rats with subcutaneously implanted growth hormone-producing tumors .
	manualset3
148188	3	409764	5	NULL	NULL	0	NULL	growth hormone levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of chronic elevations of growth hormone levels on hepatic insulin binding and action were studied in rats with subcutaneously implanted growth hormone-producing tumors .
	manualset3
148189	4	409764	5	NULL	NULL	0	NULL	hepatic insulin binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of chronic elevations of growth hormone levels on hepatic insulin binding and action were studied in rats with subcutaneously implanted growth hormone-producing tumors .
	manualset3
148190	5	409764	5	NULL	NULL	0	NULL	action 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of chronic elevations of growth hormone levels on hepatic insulin binding and action were studied in rats with subcutaneously implanted growth hormone-producing tumors .
	manualset3
148191	6	409764	5	NULL	NULL	0	NULL	rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of chronic elevations of growth hormone levels on hepatic insulin binding and action were studied in rats with subcutaneously implanted growth hormone-producing tumors .
	manualset3
148192	7	409764	5	NULL	NULL	0	NULL	growth hormone-producing tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of chronic elevations of growth hormone levels on hepatic insulin binding and action were studied in rats with subcutaneously implanted growth hormone-producing tumors .
	manualset3
148193	1	409765	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of complete fimbria-fornix ( FF ) lesioning , bilateral medial-FF lesioning and systemic administration of a novel noradrenergic alpha 2-antagonist , atipamezole , on electrophysiological properties of the hippocampal formation were studied in the rat .
	manualset3
148194	2	409765	5	NULL	NULL	0	NULL	fimbria-fornix ( FF ) lesioning 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of complete fimbria-fornix ( FF ) lesioning , bilateral medial-FF lesioning and systemic administration of a novel noradrenergic alpha 2-antagonist , atipamezole , on electrophysiological properties of the hippocampal formation were studied in the rat .
	manualset3
148195	3	409765	5	NULL	NULL	0	NULL	bilateral medial-FF lesioning	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of complete fimbria-fornix ( FF ) lesioning , bilateral medial-FF lesioning and systemic administration of a novel noradrenergic alpha 2-antagonist , atipamezole , on electrophysiological properties of the hippocampal formation were studied in the rat .
	manualset3
148196	4	409765	5	NULL	NULL	0	NULL	systemic administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of complete fimbria-fornix ( FF ) lesioning , bilateral medial-FF lesioning and systemic administration of a novel noradrenergic alpha 2-antagonist , atipamezole , on electrophysiological properties of the hippocampal formation were studied in the rat .
	manualset3
148197	5	409765	5	NULL	NULL	0	NULL	novel noradrenergic alpha 2-antagonist , atipamezole 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of complete fimbria-fornix ( FF ) lesioning , bilateral medial-FF lesioning and systemic administration of a novel noradrenergic alpha 2-antagonist , atipamezole , on electrophysiological properties of the hippocampal formation were studied in the rat .
	manualset3
148198	6	409765	5	NULL	NULL	0	NULL	electrophysiological properties 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of complete fimbria-fornix ( FF ) lesioning , bilateral medial-FF lesioning and systemic administration of a novel noradrenergic alpha 2-antagonist , atipamezole , on electrophysiological properties of the hippocampal formation were studied in the rat .
	manualset3
148199	7	409765	5	NULL	NULL	0	NULL	hippocampal formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of complete fimbria-fornix ( FF ) lesioning , bilateral medial-FF lesioning and systemic administration of a novel noradrenergic alpha 2-antagonist , atipamezole , on electrophysiological properties of the hippocampal formation were studied in the rat .
	manualset3
148200	8	409765	5	NULL	NULL	0	NULL	rat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of complete fimbria-fornix ( FF ) lesioning , bilateral medial-FF lesioning and systemic administration of a novel noradrenergic alpha 2-antagonist , atipamezole , on electrophysiological properties of the hippocampal formation were studied in the rat .
	manualset3
148201	1	409766	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of cyc2 mutations are more pronounced in rho - strains than in rho + strains , even though rho - strains that are CYC2 + contain normal levels of holocytochrome c. cyc2 mutations affect levels of iso-1-cytochrome c more than they do levels of iso-2-cytochrome c , apparently because of the greater susceptibility of apo-iso-1-cytochrome c to degradation in the cytoplasm .
	manualset3
148202	2	409766	5	NULL	NULL	0	NULL	cyc2 mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of cyc2 mutations are more pronounced in rho - strains than in rho + strains , even though rho - strains that are CYC2 + contain normal levels of holocytochrome c. cyc2 mutations affect levels of iso-1-cytochrome c more than they do levels of iso-2-cytochrome c , apparently because of the greater susceptibility of apo-iso-1-cytochrome c to degradation in the cytoplasm .
	manualset3
148203	3	409766	5	NULL	NULL	0	NULL	rho - strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of cyc2 mutations are more pronounced in rho - strains than in rho + strains , even though rho - strains that are CYC2 + contain normal levels of holocytochrome c. cyc2 mutations affect levels of iso-1-cytochrome c more than they do levels of iso-2-cytochrome c , apparently because of the greater susceptibility of apo-iso-1-cytochrome c to degradation in the cytoplasm .
	manualset3
148204	4	409766	5	NULL	NULL	0	NULL	 rho + strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of cyc2 mutations are more pronounced in rho - strains than in rho + strains , even though rho - strains that are CYC2 + contain normal levels of holocytochrome c. cyc2 mutations affect levels of iso-1-cytochrome c more than they do levels of iso-2-cytochrome c , apparently because of the greater susceptibility of apo-iso-1-cytochrome c to degradation in the cytoplasm .
	manualset3
148205	5	409766	5	NULL	NULL	NULL	NULL	rho - strains that are CYC2 +	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The effects of cyc2 mutations are more pronounced in rho - strains than in rho + strains , even though rho - strains that are CYC2 + contain normal levels of holocytochrome c. cyc2 mutations affect levels of iso-1-cytochrome c more than they do levels of iso-2-cytochrome c , apparently because of the greater susceptibility of apo-iso-1-cytochrome c to degradation in the cytoplasm .
	manualset3
148206	6	409766	5	NULL	NULL	0	NULL	normal levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of cyc2 mutations are more pronounced in rho - strains than in rho + strains , even though rho - strains that are CYC2 + contain normal levels of holocytochrome c. cyc2 mutations affect levels of iso-1-cytochrome c more than they do levels of iso-2-cytochrome c , apparently because of the greater susceptibility of apo-iso-1-cytochrome c to degradation in the cytoplasm .
	manualset3
148207	7	409766	5	NULL	NULL	NULL	NULL	holocytochrome c	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The effects of cyc2 mutations are more pronounced in rho - strains than in rho + strains , even though rho - strains that are CYC2 + contain normal levels of holocytochrome c. cyc2 mutations affect levels of iso-1-cytochrome c more than they do levels of iso-2-cytochrome c , apparently because of the greater susceptibility of apo-iso-1-cytochrome c to degradation in the cytoplasm .
	manualset3
148208	8	409766	5	NULL	NULL	0	NULL	cyc2 mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of cyc2 mutations are more pronounced in rho - strains than in rho + strains , even though rho - strains that are CYC2 + contain normal levels of holocytochrome c. cyc2 mutations affect levels of iso-1-cytochrome c more than they do levels of iso-2-cytochrome c , apparently because of the greater susceptibility of apo-iso-1-cytochrome c to degradation in the cytoplasm .
	manualset3
148209	9	409766	5	NULL	NULL	0	NULL	levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of cyc2 mutations are more pronounced in rho - strains than in rho + strains , even though rho - strains that are CYC2 + contain normal levels of holocytochrome c. cyc2 mutations affect levels of iso-1-cytochrome c more than they do levels of iso-2-cytochrome c , apparently because of the greater susceptibility of apo-iso-1-cytochrome c to degradation in the cytoplasm .
	manualset3
148210	10	409766	5	NULL	NULL	0	NULL	iso-1-cytochrome c 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of cyc2 mutations are more pronounced in rho - strains than in rho + strains , even though rho - strains that are CYC2 + contain normal levels of holocytochrome c. cyc2 mutations affect levels of iso-1-cytochrome c more than they do levels of iso-2-cytochrome c , apparently because of the greater susceptibility of apo-iso-1-cytochrome c to degradation in the cytoplasm .
	manualset3
148211	11	409766	5	NULL	NULL	0	NULL	 iso-2-cytochrome c 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of cyc2 mutations are more pronounced in rho - strains than in rho + strains , even though rho - strains that are CYC2 + contain normal levels of holocytochrome c. cyc2 mutations affect levels of iso-1-cytochrome c more than they do levels of iso-2-cytochrome c , apparently because of the greater susceptibility of apo-iso-1-cytochrome c to degradation in the cytoplasm .
	manualset3
148212	12	409766	5	NULL	NULL	0	NULL	susceptibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of cyc2 mutations are more pronounced in rho - strains than in rho + strains , even though rho - strains that are CYC2 + contain normal levels of holocytochrome c. cyc2 mutations affect levels of iso-1-cytochrome c more than they do levels of iso-2-cytochrome c , apparently because of the greater susceptibility of apo-iso-1-cytochrome c to degradation in the cytoplasm .
	manualset3
148213	13	409766	5	NULL	NULL	0	NULL	apo-iso-1-cytochrome c 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of cyc2 mutations are more pronounced in rho - strains than in rho + strains , even though rho - strains that are CYC2 + contain normal levels of holocytochrome c. cyc2 mutations affect levels of iso-1-cytochrome c more than they do levels of iso-2-cytochrome c , apparently because of the greater susceptibility of apo-iso-1-cytochrome c to degradation in the cytoplasm .
	manualset3
148214	14	409766	5	NULL	NULL	0	NULL	degradation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of cyc2 mutations are more pronounced in rho - strains than in rho + strains , even though rho - strains that are CYC2 + contain normal levels of holocytochrome c. cyc2 mutations affect levels of iso-1-cytochrome c more than they do levels of iso-2-cytochrome c , apparently because of the greater susceptibility of apo-iso-1-cytochrome c to degradation in the cytoplasm .
	manualset3
148215	15	409766	5	NULL	NULL	0	NULL	cytoplasm 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of cyc2 mutations are more pronounced in rho - strains than in rho + strains , even though rho - strains that are CYC2 + contain normal levels of holocytochrome c. cyc2 mutations affect levels of iso-1-cytochrome c more than they do levels of iso-2-cytochrome c , apparently because of the greater susceptibility of apo-iso-1-cytochrome c to degradation in the cytoplasm .
	manualset3
148216	1	409767	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of cyclophosphamide on eruption of the continuously growing mandibular incisor of the rat .
	manualset3
148217	2	409767	5	NULL	NULL	0	NULL	cyclophosphamide 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of cyclophosphamide on eruption of the continuously growing mandibular incisor of the rat .
	manualset3
148218	3	409767	5	NULL	NULL	0	NULL	eruption 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of cyclophosphamide on eruption of the continuously growing mandibular incisor of the rat .
	manualset3
148219	4	409767	5	NULL	NULL	0	NULL	mandibular incisor	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of cyclophosphamide on eruption of the continuously growing mandibular incisor of the rat .
	manualset3
148220	5	409767	5	NULL	NULL	0	NULL	rat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of cyclophosphamide on eruption of the continuously growing mandibular incisor of the rat .
	manualset3
148221	1	409768	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of different concentrations of soil cadmium ( 0 , 1 , 3 , 5 , 10 , and 20mgkg ( -1 ) ) on growth , structural changes and cadmium cellular localization in leaves of maize plants ( Zea mays L. ) were investigated in a pot experiment .
	manualset3
148222	2	409768	5	NULL	NULL	0	NULL	concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of different concentrations of soil cadmium ( 0 , 1 , 3 , 5 , 10 , and 20mgkg ( -1 ) ) on growth , structural changes and cadmium cellular localization in leaves of maize plants ( Zea mays L. ) were investigated in a pot experiment .
	manualset3
148223	3	409768	5	NULL	NULL	0	NULL	soil cadmium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of different concentrations of soil cadmium ( 0 , 1 , 3 , 5 , 10 , and 20mgkg ( -1 ) ) on growth , structural changes and cadmium cellular localization in leaves of maize plants ( Zea mays L. ) were investigated in a pot experiment .
	manualset3
148224	4	409768	5	NULL	NULL	0	NULL	 0 , 1 , 3 , 5 , 10 , and 20mgkg ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of different concentrations of soil cadmium ( 0 , 1 , 3 , 5 , 10 , and 20mgkg ( -1 ) ) on growth , structural changes and cadmium cellular localization in leaves of maize plants ( Zea mays L. ) were investigated in a pot experiment .
	manualset3
148225	5	409768	5	NULL	NULL	0	NULL	growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of different concentrations of soil cadmium ( 0 , 1 , 3 , 5 , 10 , and 20mgkg ( -1 ) ) on growth , structural changes and cadmium cellular localization in leaves of maize plants ( Zea mays L. ) were investigated in a pot experiment .
	manualset3
148226	6	409768	5	NULL	NULL	0	NULL	structural changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of different concentrations of soil cadmium ( 0 , 1 , 3 , 5 , 10 , and 20mgkg ( -1 ) ) on growth , structural changes and cadmium cellular localization in leaves of maize plants ( Zea mays L. ) were investigated in a pot experiment .
	manualset3
148227	7	409768	5	NULL	NULL	0	NULL	cadmium cellular localization 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of different concentrations of soil cadmium ( 0 , 1 , 3 , 5 , 10 , and 20mgkg ( -1 ) ) on growth , structural changes and cadmium cellular localization in leaves of maize plants ( Zea mays L. ) were investigated in a pot experiment .
	manualset3
148228	8	409768	5	NULL	NULL	0	NULL	leaves 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of different concentrations of soil cadmium ( 0 , 1 , 3 , 5 , 10 , and 20mgkg ( -1 ) ) on growth , structural changes and cadmium cellular localization in leaves of maize plants ( Zea mays L. ) were investigated in a pot experiment .
	manualset3
148229	9	409768	5	NULL	NULL	0	NULL	maize plants ( Zea mays L. )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of different concentrations of soil cadmium ( 0 , 1 , 3 , 5 , 10 , and 20mgkg ( -1 ) ) on growth , structural changes and cadmium cellular localization in leaves of maize plants ( Zea mays L. ) were investigated in a pot experiment .
	manualset3
148230	10	409768	5	NULL	NULL	0	NULL	pot experiment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of different concentrations of soil cadmium ( 0 , 1 , 3 , 5 , 10 , and 20mgkg ( -1 ) ) on growth , structural changes and cadmium cellular localization in leaves of maize plants ( Zea mays L. ) were investigated in a pot experiment .
	manualset3
148231	1	409769	5	NULL	NULL	0	NULL	steady state 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A steady state of the fermentation was maintained for the duration of more than 110 h. The dilution rate was kept in the range of 0.035 and 0.043 h ( -1 ) , and the 2KGA productivity was 3.90 to 4.80 g/L/h .
	manualset3
148232	2	409769	5	NULL	NULL	0	NULL	fermentation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A steady state of the fermentation was maintained for the duration of more than 110 h. The dilution rate was kept in the range of 0.035 and 0.043 h ( -1 ) , and the 2KGA productivity was 3.90 to 4.80 g/L/h .
	manualset3
148233	4	409769	5	NULL	NULL	NULL	NULL	110 h	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A steady state of the fermentation was maintained for the duration of more than 110 h. The dilution rate was kept in the range of 0.035 and 0.043 h ( -1 ) , and the 2KGA productivity was 3.90 to 4.80 g/L/h .
	manualset3
148234	3	409769	5	NULL	NULL	0	NULL	duration 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A steady state of the fermentation was maintained for the duration of more than 110 h. The dilution rate was kept in the range of 0.035 and 0.043 h ( -1 ) , and the 2KGA productivity was 3.90 to 4.80 g/L/h .
	manualset3
148235	5	409769	5	NULL	NULL	0	NULL	dilution rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A steady state of the fermentation was maintained for the duration of more than 110 h. The dilution rate was kept in the range of 0.035 and 0.043 h ( -1 ) , and the 2KGA productivity was 3.90 to 4.80 g/L/h .
	manualset3
148236	6	409769	5	NULL	NULL	0	NULL	range 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A steady state of the fermentation was maintained for the duration of more than 110 h. The dilution rate was kept in the range of 0.035 and 0.043 h ( -1 ) , and the 2KGA productivity was 3.90 to 4.80 g/L/h .
	manualset3
148237	7	409769	5	NULL	NULL	0	NULL	0.035 and 0.043 h ( -1 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A steady state of the fermentation was maintained for the duration of more than 110 h. The dilution rate was kept in the range of 0.035 and 0.043 h ( -1 ) , and the 2KGA productivity was 3.90 to 4.80 g/L/h .
	manualset3
148238	8	409769	5	NULL	NULL	0	NULL	2KGA productivity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A steady state of the fermentation was maintained for the duration of more than 110 h. The dilution rate was kept in the range of 0.035 and 0.043 h ( -1 ) , and the 2KGA productivity was 3.90 to 4.80 g/L/h .
	manualset3
148239	9	409769	5	NULL	NULL	0	NULL	3.90 to 4.80 g/L/h	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A steady state of the fermentation was maintained for the duration of more than 110 h. The dilution rate was kept in the range of 0.035 and 0.043 h ( -1 ) , and the 2KGA productivity was 3.90 to 4.80 g/L/h .
	manualset3
148240	1	409770	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of dopaminergic agents with different mechanisms of action in this paradigm have revealed several interesting dissociations suggesting that a rewarding signal at dopamine D1-like receptors may mediate both the acquisition of rewarding properties by neutral stimuli and their ability to control behavior .
	manualset3
148241	2	409770	5	NULL	NULL	0	NULL	dopaminergic agents	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of dopaminergic agents with different mechanisms of action in this paradigm have revealed several interesting dissociations suggesting that a rewarding signal at dopamine D1-like receptors may mediate both the acquisition of rewarding properties by neutral stimuli and their ability to control behavior .
	manualset3
148242	3	409770	5	NULL	NULL	0	NULL	mechanisms of action 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of dopaminergic agents with different mechanisms of action in this paradigm have revealed several interesting dissociations suggesting that a rewarding signal at dopamine D1-like receptors may mediate both the acquisition of rewarding properties by neutral stimuli and their ability to control behavior .
	manualset3
148243	4	409770	5	NULL	NULL	0	NULL	paradigm 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of dopaminergic agents with different mechanisms of action in this paradigm have revealed several interesting dissociations suggesting that a rewarding signal at dopamine D1-like receptors may mediate both the acquisition of rewarding properties by neutral stimuli and their ability to control behavior .
	manualset3
148244	5	409770	5	NULL	NULL	0	NULL	dissociations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of dopaminergic agents with different mechanisms of action in this paradigm have revealed several interesting dissociations suggesting that a rewarding signal at dopamine D1-like receptors may mediate both the acquisition of rewarding properties by neutral stimuli and their ability to control behavior .
	manualset3
148245	6	409770	5	NULL	NULL	0	NULL	rewarding signal	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of dopaminergic agents with different mechanisms of action in this paradigm have revealed several interesting dissociations suggesting that a rewarding signal at dopamine D1-like receptors may mediate both the acquisition of rewarding properties by neutral stimuli and their ability to control behavior .
	manualset3
148246	7	409770	5	NULL	NULL	0	NULL	dopamine D1-like receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of dopaminergic agents with different mechanisms of action in this paradigm have revealed several interesting dissociations suggesting that a rewarding signal at dopamine D1-like receptors may mediate both the acquisition of rewarding properties by neutral stimuli and their ability to control behavior .
	manualset3
148247	8	409770	5	NULL	NULL	0	NULL	acquisition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of dopaminergic agents with different mechanisms of action in this paradigm have revealed several interesting dissociations suggesting that a rewarding signal at dopamine D1-like receptors may mediate both the acquisition of rewarding properties by neutral stimuli and their ability to control behavior .
	manualset3
148248	9	409770	5	NULL	NULL	0	NULL	rewarding properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of dopaminergic agents with different mechanisms of action in this paradigm have revealed several interesting dissociations suggesting that a rewarding signal at dopamine D1-like receptors may mediate both the acquisition of rewarding properties by neutral stimuli and their ability to control behavior .
	manualset3
148249	10	409770	5	NULL	NULL	0	NULL	neutral stimuli	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of dopaminergic agents with different mechanisms of action in this paradigm have revealed several interesting dissociations suggesting that a rewarding signal at dopamine D1-like receptors may mediate both the acquisition of rewarding properties by neutral stimuli and their ability to control behavior .
	manualset3
148250	11	409770	5	NULL	NULL	0	NULL	behavior 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of dopaminergic agents with different mechanisms of action in this paradigm have revealed several interesting dissociations suggesting that a rewarding signal at dopamine D1-like receptors may mediate both the acquisition of rewarding properties by neutral stimuli and their ability to control behavior .
	manualset3
148251	1	409771	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of exogenous and endogenous superoxide on the superoxide-susceptible channels are discussed .
	manualset3
148252	2	409771	5	NULL	NULL	0	NULL	exogenous superoxide 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of exogenous and endogenous superoxide on the superoxide-susceptible channels are discussed .
	manualset3
148253	3	409771	5	NULL	NULL	0	NULL	 endogenous superoxide 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of exogenous and endogenous superoxide on the superoxide-susceptible channels are discussed .
	manualset3
148254	4	409771	5	NULL	NULL	0	NULL	 endogenous superoxide 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of exogenous and endogenous superoxide on the superoxide-susceptible channels are discussed .
	manualset3
148255	1	409772	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of forced swimming stress ( 15 minutes per day ) on body weight , food intake , blood sugar , water intake , and urine output were studied in adult male Wistar rats on the first , seventh , fourteenth and 21st days in different subgroups .
	manualset3
148256	2	409772	5	NULL	NULL	0	NULL	forced swimming stress	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of forced swimming stress ( 15 minutes per day ) on body weight , food intake , blood sugar , water intake , and urine output were studied in adult male Wistar rats on the first , seventh , fourteenth and 21st days in different subgroups .
	manualset3
148257	3	409772	5	NULL	NULL	0	NULL	15 minutes per day	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of forced swimming stress ( 15 minutes per day ) on body weight , food intake , blood sugar , water intake , and urine output were studied in adult male Wistar rats on the first , seventh , fourteenth and 21st days in different subgroups .
	manualset3
148258	4	409772	5	NULL	NULL	0	NULL	body weight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of forced swimming stress ( 15 minutes per day ) on body weight , food intake , blood sugar , water intake , and urine output were studied in adult male Wistar rats on the first , seventh , fourteenth and 21st days in different subgroups .
	manualset3
148259	5	409772	5	NULL	NULL	0	NULL	food intake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of forced swimming stress ( 15 minutes per day ) on body weight , food intake , blood sugar , water intake , and urine output were studied in adult male Wistar rats on the first , seventh , fourteenth and 21st days in different subgroups .
	manualset3
148260	6	409772	5	NULL	NULL	0	NULL	blood sugar	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of forced swimming stress ( 15 minutes per day ) on body weight , food intake , blood sugar , water intake , and urine output were studied in adult male Wistar rats on the first , seventh , fourteenth and 21st days in different subgroups .
	manualset3
148261	7	409772	5	NULL	NULL	0	NULL	water intake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of forced swimming stress ( 15 minutes per day ) on body weight , food intake , blood sugar , water intake , and urine output were studied in adult male Wistar rats on the first , seventh , fourteenth and 21st days in different subgroups .
	manualset3
148262	8	409772	5	NULL	NULL	0	NULL	urine output 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of forced swimming stress ( 15 minutes per day ) on body weight , food intake , blood sugar , water intake , and urine output were studied in adult male Wistar rats on the first , seventh , fourteenth and 21st days in different subgroups .
	manualset3
148263	9	409772	5	NULL	NULL	0	NULL	adult male Wistar rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of forced swimming stress ( 15 minutes per day ) on body weight , food intake , blood sugar , water intake , and urine output were studied in adult male Wistar rats on the first , seventh , fourteenth and 21st days in different subgroups .
	manualset3
148264	10	409772	5	NULL	NULL	0	NULL	first , seventh , fourteenth and 21st days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of forced swimming stress ( 15 minutes per day ) on body weight , food intake , blood sugar , water intake , and urine output were studied in adult male Wistar rats on the first , seventh , fourteenth and 21st days in different subgroups .
	manualset3
148265	11	409772	5	NULL	NULL	0	NULL	subgroups 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of forced swimming stress ( 15 minutes per day ) on body weight , food intake , blood sugar , water intake , and urine output were studied in adult male Wistar rats on the first , seventh , fourteenth and 21st days in different subgroups .
	manualset3
148266	1	409773	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of four calcium entry blockers ( CEBs ) , diltiazem ( D ) , verapamil ( V ) , nifedipine ( NF ) and nicardipine ( NC ) , were investigated on Ca2 + concentration-effect curves of rat depolarized ( K + , 40 mM ) or noradrenaline ( NA , 3 microM ) - exposed mesenteric resistance vessels .
	manualset3
148267	2	409773	5	NULL	NULL	0	NULL	four 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of four calcium entry blockers ( CEBs ) , diltiazem ( D ) , verapamil ( V ) , nifedipine ( NF ) and nicardipine ( NC ) , were investigated on Ca2 + concentration-effect curves of rat depolarized ( K + , 40 mM ) or noradrenaline ( NA , 3 microM ) - exposed mesenteric resistance vessels .
	manualset3
148268	3	409773	5	NULL	NULL	NULL	NULL	calcium entry blockers ( CEBs )	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The effects of four calcium entry blockers ( CEBs ) , diltiazem ( D ) , verapamil ( V ) , nifedipine ( NF ) and nicardipine ( NC ) , were investigated on Ca2 + concentration-effect curves of rat depolarized ( K + , 40 mM ) or noradrenaline ( NA , 3 microM ) - exposed mesenteric resistance vessels .
	manualset3
148269	4	409773	5	NULL	NULL	0	NULL	diltiazem ( D )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of four calcium entry blockers ( CEBs ) , diltiazem ( D ) , verapamil ( V ) , nifedipine ( NF ) and nicardipine ( NC ) , were investigated on Ca2 + concentration-effect curves of rat depolarized ( K + , 40 mM ) or noradrenaline ( NA , 3 microM ) - exposed mesenteric resistance vessels .
	manualset3
148270	5	409773	5	NULL	NULL	0	NULL	verapamil ( V )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of four calcium entry blockers ( CEBs ) , diltiazem ( D ) , verapamil ( V ) , nifedipine ( NF ) and nicardipine ( NC ) , were investigated on Ca2 + concentration-effect curves of rat depolarized ( K + , 40 mM ) or noradrenaline ( NA , 3 microM ) - exposed mesenteric resistance vessels .
	manualset3
148271	6	409773	5	NULL	NULL	NULL	NULL	nifedipine ( NF ) 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The effects of four calcium entry blockers ( CEBs ) , diltiazem ( D ) , verapamil ( V ) , nifedipine ( NF ) and nicardipine ( NC ) , were investigated on Ca2 + concentration-effect curves of rat depolarized ( K + , 40 mM ) or noradrenaline ( NA , 3 microM ) - exposed mesenteric resistance vessels .
	manualset3
148272	7	409773	5	NULL	NULL	0	NULL	nicardipine ( NC )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of four calcium entry blockers ( CEBs ) , diltiazem ( D ) , verapamil ( V ) , nifedipine ( NF ) and nicardipine ( NC ) , were investigated on Ca2 + concentration-effect curves of rat depolarized ( K + , 40 mM ) or noradrenaline ( NA , 3 microM ) - exposed mesenteric resistance vessels .
	manualset3
148273	8	409773	5	NULL	NULL	0	NULL	Ca2 + concentration-effect curves	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of four calcium entry blockers ( CEBs ) , diltiazem ( D ) , verapamil ( V ) , nifedipine ( NF ) and nicardipine ( NC ) , were investigated on Ca2 + concentration-effect curves of rat depolarized ( K + , 40 mM ) or noradrenaline ( NA , 3 microM ) - exposed mesenteric resistance vessels .
	manualset3
148274	9	409773	5	NULL	NULL	0	NULL	rat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of four calcium entry blockers ( CEBs ) , diltiazem ( D ) , verapamil ( V ) , nifedipine ( NF ) and nicardipine ( NC ) , were investigated on Ca2 + concentration-effect curves of rat depolarized ( K + , 40 mM ) or noradrenaline ( NA , 3 microM ) - exposed mesenteric resistance vessels .
	manualset3
148275	10	409773	5	NULL	NULL	0	NULL	K +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of four calcium entry blockers ( CEBs ) , diltiazem ( D ) , verapamil ( V ) , nifedipine ( NF ) and nicardipine ( NC ) , were investigated on Ca2 + concentration-effect curves of rat depolarized ( K + , 40 mM ) or noradrenaline ( NA , 3 microM ) - exposed mesenteric resistance vessels .
	manualset3
148276	11	409773	5	NULL	NULL	0	NULL	40 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of four calcium entry blockers ( CEBs ) , diltiazem ( D ) , verapamil ( V ) , nifedipine ( NF ) and nicardipine ( NC ) , were investigated on Ca2 + concentration-effect curves of rat depolarized ( K + , 40 mM ) or noradrenaline ( NA , 3 microM ) - exposed mesenteric resistance vessels .
	manualset3
148277	12	409773	5	NULL	NULL	0	NULL	noradrenaline ( NA , 3 microM ) - exposed mesenteric resistance vessels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of four calcium entry blockers ( CEBs ) , diltiazem ( D ) , verapamil ( V ) , nifedipine ( NF ) and nicardipine ( NC ) , were investigated on Ca2 + concentration-effect curves of rat depolarized ( K + , 40 mM ) or noradrenaline ( NA , 3 microM ) - exposed mesenteric resistance vessels .
	manualset3
148278	1	409774	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of gammahydroxybutyrate on hypermetabolism and wound healing in a rat model of large thermal injury .
	manualset3
148279	2	409774	5	NULL	NULL	0	NULL	gammahydroxybutyrate 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of gammahydroxybutyrate on hypermetabolism and wound healing in a rat model of large thermal injury .
	manualset3
148280	3	409774	5	NULL	NULL	NULL	NULL	hypermetabolism 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The effects of gammahydroxybutyrate on hypermetabolism and wound healing in a rat model of large thermal injury .
	manualset3
148281	4	409774	5	NULL	NULL	0	NULL	wound healing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of gammahydroxybutyrate on hypermetabolism and wound healing in a rat model of large thermal injury .
	manualset3
148282	5	409774	5	NULL	NULL	0	NULL	rat model	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of gammahydroxybutyrate on hypermetabolism and wound healing in a rat model of large thermal injury .
	manualset3
148283	6	409774	5	NULL	NULL	0	NULL	thermal injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of gammahydroxybutyrate on hypermetabolism and wound healing in a rat model of large thermal injury .
	manualset3
148284	1	409775	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of in vivo modulation of murine collagen induced arthritis with monoclonal anti-CD4 antibodies , monoclonal anti-Ia antibodies , and gamma interferon are reviewed .
	manualset3
148285	2	409775	5	NULL	NULL	0	NULL	modulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of in vivo modulation of murine collagen induced arthritis with monoclonal anti-CD4 antibodies , monoclonal anti-Ia antibodies , and gamma interferon are reviewed .
	manualset3
148286	3	409775	5	NULL	NULL	0	NULL	murine collagen induced arthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of in vivo modulation of murine collagen induced arthritis with monoclonal anti-CD4 antibodies , monoclonal anti-Ia antibodies , and gamma interferon are reviewed .
	manualset3
148287	4	409775	5	NULL	NULL	0	NULL	monoclonal anti-CD4 antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of in vivo modulation of murine collagen induced arthritis with monoclonal anti-CD4 antibodies , monoclonal anti-Ia antibodies , and gamma interferon are reviewed .
	manualset3
148288	5	409775	5	NULL	NULL	0	NULL	monoclonal anti-Ia antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of in vivo modulation of murine collagen induced arthritis with monoclonal anti-CD4 antibodies , monoclonal anti-Ia antibodies , and gamma interferon are reviewed .
	manualset3
148289	6	409775	5	NULL	NULL	0	NULL	gamma interferon	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of in vivo modulation of murine collagen induced arthritis with monoclonal anti-CD4 antibodies , monoclonal anti-Ia antibodies , and gamma interferon are reviewed .
	manualset3
148290	1	409776	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of increasing the level of cyclic AMP ( cAMP ) activity on lymphocyte proliferation in the rat mixed lymphocyte reaction ( MLR ) were investigated .
	manualset3
148291	2	409776	5	NULL	NULL	0	NULL	level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of increasing the level of cyclic AMP ( cAMP ) activity on lymphocyte proliferation in the rat mixed lymphocyte reaction ( MLR ) were investigated .
	manualset3
148292	3	409776	5	NULL	NULL	0	NULL	cyclic AMP ( cAMP ) activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of increasing the level of cyclic AMP ( cAMP ) activity on lymphocyte proliferation in the rat mixed lymphocyte reaction ( MLR ) were investigated .
	manualset3
148293	4	409776	5	NULL	NULL	0	NULL	lymphocyte proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of increasing the level of cyclic AMP ( cAMP ) activity on lymphocyte proliferation in the rat mixed lymphocyte reaction ( MLR ) were investigated .
	manualset3
148294	5	409776	5	NULL	NULL	0	NULL	rat mixed lymphocyte reaction ( MLR )	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of increasing the level of cyclic AMP ( cAMP ) activity on lymphocyte proliferation in the rat mixed lymphocyte reaction ( MLR ) were investigated .
	manualset3
148295	1	409777	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of inhalation of such pollutant gases on platelet function and blood viscosity have not been sufficiently investigated , even if these parameters seem to be in strict correlation with cardiovascular function .
	manualset3
148296	2	409777	5	NULL	NULL	0	NULL	inhalation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of inhalation of such pollutant gases on platelet function and blood viscosity have not been sufficiently investigated , even if these parameters seem to be in strict correlation with cardiovascular function .
	manualset3
148297	3	409777	5	NULL	NULL	0	NULL	pollutant gases	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of inhalation of such pollutant gases on platelet function and blood viscosity have not been sufficiently investigated , even if these parameters seem to be in strict correlation with cardiovascular function .
	manualset3
148298	4	409777	5	NULL	NULL	0	NULL	platelet function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of inhalation of such pollutant gases on platelet function and blood viscosity have not been sufficiently investigated , even if these parameters seem to be in strict correlation with cardiovascular function .
	manualset3
148299	5	409777	5	NULL	NULL	0	NULL	blood viscosity	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of inhalation of such pollutant gases on platelet function and blood viscosity have not been sufficiently investigated , even if these parameters seem to be in strict correlation with cardiovascular function .
	manualset3
148300	6	409777	5	NULL	NULL	0	NULL	parameters 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of inhalation of such pollutant gases on platelet function and blood viscosity have not been sufficiently investigated , even if these parameters seem to be in strict correlation with cardiovascular function .
	manualset3
148301	7	409777	5	NULL	NULL	0	NULL	correlation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of inhalation of such pollutant gases on platelet function and blood viscosity have not been sufficiently investigated , even if these parameters seem to be in strict correlation with cardiovascular function .
	manualset3
148302	8	409777	5	NULL	NULL	0	NULL	cardiovascular function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of inhalation of such pollutant gases on platelet function and blood viscosity have not been sufficiently investigated , even if these parameters seem to be in strict correlation with cardiovascular function .
	manualset3
148303	1	409778	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of inhibiting nitric oxide ( NO ) synthase with NG-nitro-L-arginine ( L-NNA ) on renal vasoconstrictor responses to intrarenally administered norepinephrine ( NE ) and endothelin-1 ( ET-1 ) were studied in conscious dogs .
	manualset3
148304	2	409778	5	NULL	NULL	0	NULL	nitric oxide ( NO ) synthase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of inhibiting nitric oxide ( NO ) synthase with NG-nitro-L-arginine ( L-NNA ) on renal vasoconstrictor responses to intrarenally administered norepinephrine ( NE ) and endothelin-1 ( ET-1 ) were studied in conscious dogs .
	manualset3
148305	3	409778	5	NULL	NULL	0	NULL	NG-nitro-L-arginine ( L-NNA )	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of inhibiting nitric oxide ( NO ) synthase with NG-nitro-L-arginine ( L-NNA ) on renal vasoconstrictor responses to intrarenally administered norepinephrine ( NE ) and endothelin-1 ( ET-1 ) were studied in conscious dogs .
	manualset3
148306	4	409778	5	NULL	NULL	0	NULL	renal vasoconstrictor responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of inhibiting nitric oxide ( NO ) synthase with NG-nitro-L-arginine ( L-NNA ) on renal vasoconstrictor responses to intrarenally administered norepinephrine ( NE ) and endothelin-1 ( ET-1 ) were studied in conscious dogs .
	manualset3
148307	5	409778	5	NULL	NULL	0	NULL	norepinephrine ( NE )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of inhibiting nitric oxide ( NO ) synthase with NG-nitro-L-arginine ( L-NNA ) on renal vasoconstrictor responses to intrarenally administered norepinephrine ( NE ) and endothelin-1 ( ET-1 ) were studied in conscious dogs .
	manualset3
148308	6	409778	5	NULL	NULL	0	NULL	endothelin-1 ( ET-1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of inhibiting nitric oxide ( NO ) synthase with NG-nitro-L-arginine ( L-NNA ) on renal vasoconstrictor responses to intrarenally administered norepinephrine ( NE ) and endothelin-1 ( ET-1 ) were studied in conscious dogs .
	manualset3
148309	7	409778	5	NULL	NULL	0	NULL	conscious dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of inhibiting nitric oxide ( NO ) synthase with NG-nitro-L-arginine ( L-NNA ) on renal vasoconstrictor responses to intrarenally administered norepinephrine ( NE ) and endothelin-1 ( ET-1 ) were studied in conscious dogs .
	manualset3
148310	1	409779	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of intravenous infusions of triglycerides on the secretion of milk fat in the cow .
	manualset3
148311	2	409779	5	NULL	NULL	0	NULL	intravenous infusions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of intravenous infusions of triglycerides on the secretion of milk fat in the cow .
	manualset3
148312	3	409779	5	NULL	NULL	0	NULL	triglycerides 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of intravenous infusions of triglycerides on the secretion of milk fat in the cow .
	manualset3
148313	4	409779	5	NULL	NULL	0	NULL	secretion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of intravenous infusions of triglycerides on the secretion of milk fat in the cow .
	manualset3
148314	5	409779	5	NULL	NULL	0	NULL	milk fat 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of intravenous infusions of triglycerides on the secretion of milk fat in the cow .
	manualset3
148315	6	409779	5	NULL	NULL	0	NULL	cow 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of intravenous infusions of triglycerides on the secretion of milk fat in the cow .
	manualset3
148316	1	409780	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of long-term tamoxifen exposure on cell growth and cell cycle kinetics were compared between estrogen receptor ( ER ) - positive ( MCF-7 ) and ER-negative ( MDA-MB-231 ) cell lines .
	manualset3
148317	2	409780	5	NULL	NULL	0	NULL	long-term tamoxifen exposure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of long-term tamoxifen exposure on cell growth and cell cycle kinetics were compared between estrogen receptor ( ER ) - positive ( MCF-7 ) and ER-negative ( MDA-MB-231 ) cell lines .
	manualset3
148318	3	409780	5	NULL	NULL	0	NULL	cell growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of long-term tamoxifen exposure on cell growth and cell cycle kinetics were compared between estrogen receptor ( ER ) - positive ( MCF-7 ) and ER-negative ( MDA-MB-231 ) cell lines .
	manualset3
148319	4	409780	5	NULL	NULL	0	NULL	cell cycle kinetics	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of long-term tamoxifen exposure on cell growth and cell cycle kinetics were compared between estrogen receptor ( ER ) - positive ( MCF-7 ) and ER-negative ( MDA-MB-231 ) cell lines .
	manualset3
148320	5	409780	5	NULL	NULL	0	NULL	estrogen receptor ( ER ) - positive ( MCF-7 )  cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of long-term tamoxifen exposure on cell growth and cell cycle kinetics were compared between estrogen receptor ( ER ) - positive ( MCF-7 ) and ER-negative ( MDA-MB-231 ) cell lines .
	manualset3
148321	6	409780	5	NULL	NULL	0	NULL	ER-negative ( MDA-MB-231 ) cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of long-term tamoxifen exposure on cell growth and cell cycle kinetics were compared between estrogen receptor ( ER ) - positive ( MCF-7 ) and ER-negative ( MDA-MB-231 ) cell lines .
	manualset3
148322	1	409781	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of method of castration , rearing condition and diet on sensory quality of pork assessed by a trained panel .
	manualset3
148323	2	409781	5	NULL	NULL	0	NULL	method of castration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of method of castration , rearing condition and diet on sensory quality of pork assessed by a trained panel .
	manualset3
148324	3	409781	5	NULL	NULL	0	NULL	rearing condition	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of method of castration , rearing condition and diet on sensory quality of pork assessed by a trained panel .
	manualset3
148325	4	409781	5	NULL	NULL	0	NULL	diet 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of method of castration , rearing condition and diet on sensory quality of pork assessed by a trained panel .
	manualset3
148326	5	409781	5	NULL	NULL	0	NULL	sensory quality 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of method of castration , rearing condition and diet on sensory quality of pork assessed by a trained panel .
	manualset3
148327	6	409781	5	NULL	NULL	0	NULL	pork 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of method of castration , rearing condition and diet on sensory quality of pork assessed by a trained panel .
	manualset3
148328	7	409781	5	NULL	NULL	0	NULL	trained panel	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of method of castration , rearing condition and diet on sensory quality of pork assessed by a trained panel .
	manualset3
148329	1	409782	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of nucleus raphe magnus lesions on an ascending thermal pathway in the rat .
	manualset3
148330	2	409782	5	NULL	NULL	0	NULL	nucleus raphe magnus lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of nucleus raphe magnus lesions on an ascending thermal pathway in the rat .
	manualset3
148331	3	409782	5	NULL	NULL	0	NULL	ascending thermal pathway 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of nucleus raphe magnus lesions on an ascending thermal pathway in the rat .
	manualset3
148332	4	409782	5	NULL	NULL	0	NULL	rat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of nucleus raphe magnus lesions on an ascending thermal pathway in the rat .
	manualset3
148333	1	409783	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of overproducing UGPase on the cell metabolism and morphology were carbon-source dependent .
	manualset3
148334	2	409783	5	NULL	NULL	0	NULL	UGPase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of overproducing UGPase on the cell metabolism and morphology were carbon-source dependent .
	manualset3
148335	3	409783	5	NULL	NULL	0	NULL	cell metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of overproducing UGPase on the cell metabolism and morphology were carbon-source dependent .
	manualset3
148336	4	409783	5	NULL	NULL	0	NULL	morphology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of overproducing UGPase on the cell metabolism and morphology were carbon-source dependent .
	manualset3
148337	1	409784	5	NULL	NULL	NULL	NULL	effects 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The effects of paradoxical sleep deprivation on estrous cycles of the female rats .
	manualset3
148338	2	409784	5	NULL	NULL	NULL	NULL	paradoxical sleep deprivation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The effects of paradoxical sleep deprivation on estrous cycles of the female rats .
	manualset3
148339	3	409784	5	NULL	NULL	0	NULL	estrous cycles	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of paradoxical sleep deprivation on estrous cycles of the female rats .
	manualset3
148340	4	409784	5	NULL	NULL	0	NULL	female rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of paradoxical sleep deprivation on estrous cycles of the female rats .
	manualset3
148341	1	409785	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of passive exercise therapy initiated prior to or after the development of hyperreflexia following spinal transection .
	manualset3
148342	2	409785	5	NULL	NULL	0	NULL	passive exercise therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of passive exercise therapy initiated prior to or after the development of hyperreflexia following spinal transection .
	manualset3
148343	3	409785	5	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of passive exercise therapy initiated prior to or after the development of hyperreflexia following spinal transection .
	manualset3
148344	4	409785	5	NULL	NULL	0	NULL	hyperreflexia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of passive exercise therapy initiated prior to or after the development of hyperreflexia following spinal transection .
	manualset3
148345	5	409785	5	NULL	NULL	0	NULL	spinal transection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of passive exercise therapy initiated prior to or after the development of hyperreflexia following spinal transection .
	manualset3
148346	1	409786	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of pravastatin and pioglitazone in combination on superoxide generation and procollagen-1 expression mimicked those of alpha-tocopherol and gamma-tocopherol , two potent antioxidants .
	manualset3
148347	2	409786	5	NULL	NULL	0	NULL	pravastatin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of pravastatin and pioglitazone in combination on superoxide generation and procollagen-1 expression mimicked those of alpha-tocopherol and gamma-tocopherol , two potent antioxidants .
	manualset3
148348	3	409786	5	NULL	NULL	0	NULL	pioglitazone 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of pravastatin and pioglitazone in combination on superoxide generation and procollagen-1 expression mimicked those of alpha-tocopherol and gamma-tocopherol , two potent antioxidants .
	manualset3
148349	4	409786	5	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of pravastatin and pioglitazone in combination on superoxide generation and procollagen-1 expression mimicked those of alpha-tocopherol and gamma-tocopherol , two potent antioxidants .
	manualset3
148350	5	409786	5	NULL	NULL	0	NULL	superoxide generation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of pravastatin and pioglitazone in combination on superoxide generation and procollagen-1 expression mimicked those of alpha-tocopherol and gamma-tocopherol , two potent antioxidants .
	manualset3
148351	6	409786	5	NULL	NULL	0	NULL	procollagen-1 expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of pravastatin and pioglitazone in combination on superoxide generation and procollagen-1 expression mimicked those of alpha-tocopherol and gamma-tocopherol , two potent antioxidants .
	manualset3
148352	7	409786	5	NULL	NULL	0	NULL	alpha-tocopherol 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of pravastatin and pioglitazone in combination on superoxide generation and procollagen-1 expression mimicked those of alpha-tocopherol and gamma-tocopherol , two potent antioxidants .
	manualset3
148353	8	409786	5	NULL	NULL	0	NULL	gamma-tocopherol 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of pravastatin and pioglitazone in combination on superoxide generation and procollagen-1 expression mimicked those of alpha-tocopherol and gamma-tocopherol , two potent antioxidants .
	manualset3
148354	9	409786	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of pravastatin and pioglitazone in combination on superoxide generation and procollagen-1 expression mimicked those of alpha-tocopherol and gamma-tocopherol , two potent antioxidants .
	manualset3
148355	10	409786	5	NULL	NULL	0	NULL	potent antioxidants	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of pravastatin and pioglitazone in combination on superoxide generation and procollagen-1 expression mimicked those of alpha-tocopherol and gamma-tocopherol , two potent antioxidants .
	manualset3
148356	1	409787	5	NULL	NULL	0	NULL	v	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of radiation on brain and body development were similar for both males and females .
	manualset3
148357	2	409787	5	NULL	NULL	0	NULL	radiation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of radiation on brain and body development were similar for both males and females .
	manualset3
148358	3	409787	5	NULL	NULL	0	NULL	brain development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of radiation on brain and body development were similar for both males and females .
	manualset3
148359	4	409787	5	NULL	NULL	0	NULL	body development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of radiation on brain and body development were similar for both males and females .
	manualset3
148360	5	409787	5	NULL	NULL	0	NULL	males 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of radiation on brain and body development were similar for both males and females .
	manualset3
148361	6	409787	5	NULL	NULL	0	NULL	females 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of radiation on brain and body development were similar for both males and females .
	manualset3
148362	1	409788	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of ranitidine hydrochloride , a histamine H2-receptor antagonist , on delivery , lactation , postnatal development of F1 generation of Crj : CD ( SD ) rats were examined .
	manualset3
148363	2	409788	5	NULL	NULL	0	NULL	ranitidine hydrochloride , a histamine H2-receptor antagonist 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of ranitidine hydrochloride , a histamine H2-receptor antagonist , on delivery , lactation , postnatal development of F1 generation of Crj : CD ( SD ) rats were examined .
	manualset3
148364	3	409788	5	NULL	NULL	0	NULL	delivery 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of ranitidine hydrochloride , a histamine H2-receptor antagonist , on delivery , lactation , postnatal development of F1 generation of Crj : CD ( SD ) rats were examined .
	manualset3
148365	4	409788	5	NULL	NULL	0	NULL	lactation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of ranitidine hydrochloride , a histamine H2-receptor antagonist , on delivery , lactation , postnatal development of F1 generation of Crj : CD ( SD ) rats were examined .
	manualset3
148366	5	409788	5	NULL	NULL	0	NULL	 postnatal development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of ranitidine hydrochloride , a histamine H2-receptor antagonist , on delivery , lactation , postnatal development of F1 generation of Crj : CD ( SD ) rats were examined .
	manualset3
148367	6	409788	5	NULL	NULL	0	NULL	F1 generation of Crj : CD ( SD ) rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of ranitidine hydrochloride , a histamine H2-receptor antagonist , on delivery , lactation , postnatal development of F1 generation of Crj : CD ( SD ) rats were examined .
	manualset3
148368	1	409789	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of retinoids on bone may be profound and include progressive calcification of ligaments and tendon insertions , premature fusion of epiphyses , modeling abnormalities of long bones , and perhaps osteoporosis .
	manualset3
148369	2	409789	5	NULL	NULL	0	NULL	retinoids 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of retinoids on bone may be profound and include progressive calcification of ligaments and tendon insertions , premature fusion of epiphyses , modeling abnormalities of long bones , and perhaps osteoporosis .
	manualset3
148370	3	409789	5	NULL	NULL	0	NULL	bone 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of retinoids on bone may be profound and include progressive calcification of ligaments and tendon insertions , premature fusion of epiphyses , modeling abnormalities of long bones , and perhaps osteoporosis .
	manualset3
148371	4	409789	5	NULL	NULL	0	NULL	progressive calcification 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of retinoids on bone may be profound and include progressive calcification of ligaments and tendon insertions , premature fusion of epiphyses , modeling abnormalities of long bones , and perhaps osteoporosis .
	manualset3
148372	5	409789	5	NULL	NULL	0	NULL	ligaments 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of retinoids on bone may be profound and include progressive calcification of ligaments and tendon insertions , premature fusion of epiphyses , modeling abnormalities of long bones , and perhaps osteoporosis .
	manualset3
148373	6	409789	5	NULL	NULL	0	NULL	tendon insertions	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of retinoids on bone may be profound and include progressive calcification of ligaments and tendon insertions , premature fusion of epiphyses , modeling abnormalities of long bones , and perhaps osteoporosis .
	manualset3
148374	7	409789	5	NULL	NULL	NULL	NULL	premature fusion 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The effects of retinoids on bone may be profound and include progressive calcification of ligaments and tendon insertions , premature fusion of epiphyses , modeling abnormalities of long bones , and perhaps osteoporosis .
	manualset3
148375	8	409789	5	NULL	NULL	0	NULL	epiphyses 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of retinoids on bone may be profound and include progressive calcification of ligaments and tendon insertions , premature fusion of epiphyses , modeling abnormalities of long bones , and perhaps osteoporosis .
	manualset3
148376	9	409789	5	NULL	NULL	0	NULL	modeling abnormalities 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of retinoids on bone may be profound and include progressive calcification of ligaments and tendon insertions , premature fusion of epiphyses , modeling abnormalities of long bones , and perhaps osteoporosis .
	manualset3
148377	10	409789	5	NULL	NULL	0	NULL	long bones	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of retinoids on bone may be profound and include progressive calcification of ligaments and tendon insertions , premature fusion of epiphyses , modeling abnormalities of long bones , and perhaps osteoporosis .
	manualset3
148378	11	409789	5	NULL	NULL	0	NULL	osteoporosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of retinoids on bone may be profound and include progressive calcification of ligaments and tendon insertions , premature fusion of epiphyses , modeling abnormalities of long bones , and perhaps osteoporosis .
	manualset3
148379	1	409790	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of rhIL-6 ( 500 U/ml ) were completely abolished by the preincubation of the slices with monoclonal anti-IL-6 receptor antibody ( 16 microg/ml ) for 2 h. Heat-inactivated rhIL-6 had no effect on the synaptic potentiation .
	manualset3
148380	2	409790	5	NULL	NULL	0	NULL	rhIL-6 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of rhIL-6 ( 500 U/ml ) were completely abolished by the preincubation of the slices with monoclonal anti-IL-6 receptor antibody ( 16 microg/ml ) for 2 h. Heat-inactivated rhIL-6 had no effect on the synaptic potentiation .
	manualset3
148381	3	409790	5	NULL	NULL	0	NULL	500 U/ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of rhIL-6 ( 500 U/ml ) were completely abolished by the preincubation of the slices with monoclonal anti-IL-6 receptor antibody ( 16 microg/ml ) for 2 h. Heat-inactivated rhIL-6 had no effect on the synaptic potentiation .
	manualset3
148382	4	409790	5	NULL	NULL	0	NULL	preincubation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of rhIL-6 ( 500 U/ml ) were completely abolished by the preincubation of the slices with monoclonal anti-IL-6 receptor antibody ( 16 microg/ml ) for 2 h. Heat-inactivated rhIL-6 had no effect on the synaptic potentiation .
	manualset3
148383	5	409790	5	NULL	NULL	0	NULL	slices 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of rhIL-6 ( 500 U/ml ) were completely abolished by the preincubation of the slices with monoclonal anti-IL-6 receptor antibody ( 16 microg/ml ) for 2 h. Heat-inactivated rhIL-6 had no effect on the synaptic potentiation .
	manualset3
148384	6	409790	5	NULL	NULL	0	NULL	monoclonal anti-IL-6 receptor antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of rhIL-6 ( 500 U/ml ) were completely abolished by the preincubation of the slices with monoclonal anti-IL-6 receptor antibody ( 16 microg/ml ) for 2 h. Heat-inactivated rhIL-6 had no effect on the synaptic potentiation .
	manualset3
148385	7	409790	5	NULL	NULL	0	NULL	16 microg/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of rhIL-6 ( 500 U/ml ) were completely abolished by the preincubation of the slices with monoclonal anti-IL-6 receptor antibody ( 16 microg/ml ) for 2 h. Heat-inactivated rhIL-6 had no effect on the synaptic potentiation .
	manualset3
148386	8	409790	5	NULL	NULL	0	NULL	2 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of rhIL-6 ( 500 U/ml ) were completely abolished by the preincubation of the slices with monoclonal anti-IL-6 receptor antibody ( 16 microg/ml ) for 2 h. Heat-inactivated rhIL-6 had no effect on the synaptic potentiation .
	manualset3
148387	9	409790	5	NULL	NULL	0	NULL	Heat-inactivated rhIL-6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of rhIL-6 ( 500 U/ml ) were completely abolished by the preincubation of the slices with monoclonal anti-IL-6 receptor antibody ( 16 microg/ml ) for 2 h. Heat-inactivated rhIL-6 had no effect on the synaptic potentiation .
	manualset3
148388	10	409790	5	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of rhIL-6 ( 500 U/ml ) were completely abolished by the preincubation of the slices with monoclonal anti-IL-6 receptor antibody ( 16 microg/ml ) for 2 h. Heat-inactivated rhIL-6 had no effect on the synaptic potentiation .
	manualset3
148389	11	409790	5	NULL	NULL	0	NULL	synaptic potentiation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of rhIL-6 ( 500 U/ml ) were completely abolished by the preincubation of the slices with monoclonal anti-IL-6 receptor antibody ( 16 microg/ml ) for 2 h. Heat-inactivated rhIL-6 had no effect on the synaptic potentiation .
	manualset3
148390	1	409791	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of several commonly employed fixatives on the three-dimensional conformations of two soluble proteins and the protein of intact red blood cell membranes have been studied by means of circular dichroism measurements in the spectral region of the peptide absorption bands .
	manualset3
148391	2	409791	5	NULL	NULL	0	NULL	fixatives 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of several commonly employed fixatives on the three-dimensional conformations of two soluble proteins and the protein of intact red blood cell membranes have been studied by means of circular dichroism measurements in the spectral region of the peptide absorption bands .
	manualset3
148392	3	409791	5	NULL	NULL	0	NULL	three-dimensional conformations 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of several commonly employed fixatives on the three-dimensional conformations of two soluble proteins and the protein of intact red blood cell membranes have been studied by means of circular dichroism measurements in the spectral region of the peptide absorption bands .
	manualset3
148393	4	409791	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of several commonly employed fixatives on the three-dimensional conformations of two soluble proteins and the protein of intact red blood cell membranes have been studied by means of circular dichroism measurements in the spectral region of the peptide absorption bands .
	manualset3
148394	5	409791	5	NULL	NULL	0	NULL	soluble proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of several commonly employed fixatives on the three-dimensional conformations of two soluble proteins and the protein of intact red blood cell membranes have been studied by means of circular dichroism measurements in the spectral region of the peptide absorption bands .
	manualset3
148395	6	409791	5	NULL	NULL	0	NULL	protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of several commonly employed fixatives on the three-dimensional conformations of two soluble proteins and the protein of intact red blood cell membranes have been studied by means of circular dichroism measurements in the spectral region of the peptide absorption bands .
	manualset3
148396	7	409791	5	NULL	NULL	0	NULL	red blood cell membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of several commonly employed fixatives on the three-dimensional conformations of two soluble proteins and the protein of intact red blood cell membranes have been studied by means of circular dichroism measurements in the spectral region of the peptide absorption bands .
	manualset3
148397	8	409791	5	NULL	NULL	0	NULL	circular dichroism measurements	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of several commonly employed fixatives on the three-dimensional conformations of two soluble proteins and the protein of intact red blood cell membranes have been studied by means of circular dichroism measurements in the spectral region of the peptide absorption bands .
	manualset3
148398	9	409791	5	NULL	NULL	0	NULL	spectral region	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of several commonly employed fixatives on the three-dimensional conformations of two soluble proteins and the protein of intact red blood cell membranes have been studied by means of circular dichroism measurements in the spectral region of the peptide absorption bands .
	manualset3
148399	10	409791	5	NULL	NULL	0	NULL	peptide absorption bands 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of several commonly employed fixatives on the three-dimensional conformations of two soluble proteins and the protein of intact red blood cell membranes have been studied by means of circular dichroism measurements in the spectral region of the peptide absorption bands .
	manualset3
148400	1	409792	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of shearing , pH , and ethanol concentration of beer on the particle size distribution of the highest molecular weight arabinoxylan fraction in beer were also examined .
	manualset3
148401	2	409792	5	NULL	NULL	0	NULL	shearing 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of shearing , pH , and ethanol concentration of beer on the particle size distribution of the highest molecular weight arabinoxylan fraction in beer were also examined .
	manualset3
148402	3	409792	5	NULL	NULL	0	NULL	pH 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of shearing , pH , and ethanol concentration of beer on the particle size distribution of the highest molecular weight arabinoxylan fraction in beer were also examined .
	manualset3
148403	4	409792	5	NULL	NULL	0	NULL	ethanol concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of shearing , pH , and ethanol concentration of beer on the particle size distribution of the highest molecular weight arabinoxylan fraction in beer were also examined .
	manualset3
148404	5	409792	5	NULL	NULL	0	NULL	beer 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of shearing , pH , and ethanol concentration of beer on the particle size distribution of the highest molecular weight arabinoxylan fraction in beer were also examined .
	manualset3
148405	6	409792	5	NULL	NULL	0	NULL	particle size distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of shearing , pH , and ethanol concentration of beer on the particle size distribution of the highest molecular weight arabinoxylan fraction in beer were also examined .
	manualset3
148406	7	409792	5	NULL	NULL	0	NULL	highest molecular weight arabinoxylan fraction	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of shearing , pH , and ethanol concentration of beer on the particle size distribution of the highest molecular weight arabinoxylan fraction in beer were also examined .
	manualset3
148407	8	409792	5	NULL	NULL	0	NULL	beer 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of shearing , pH , and ethanol concentration of beer on the particle size distribution of the highest molecular weight arabinoxylan fraction in beer were also examined .
	manualset3
148408	1	409793	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of sickling on cholesterol exchange between red cell membranes and serum lipoproteins were studied by following the movement of tritiated cholesterol incorporated into erythrocytes .
	manualset3
148409	2	409793	5	NULL	NULL	0	NULL	sickling 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of sickling on cholesterol exchange between red cell membranes and serum lipoproteins were studied by following the movement of tritiated cholesterol incorporated into erythrocytes .
	manualset3
148410	3	409793	5	NULL	NULL	0	NULL	cholesterol exchange	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of sickling on cholesterol exchange between red cell membranes and serum lipoproteins were studied by following the movement of tritiated cholesterol incorporated into erythrocytes .
	manualset3
148411	4	409793	5	NULL	NULL	0	NULL	red cell membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of sickling on cholesterol exchange between red cell membranes and serum lipoproteins were studied by following the movement of tritiated cholesterol incorporated into erythrocytes .
	manualset3
148412	5	409793	5	NULL	NULL	0	NULL	serum lipoproteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of sickling on cholesterol exchange between red cell membranes and serum lipoproteins were studied by following the movement of tritiated cholesterol incorporated into erythrocytes .
	manualset3
148413	6	409793	5	NULL	NULL	0	NULL	movement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of sickling on cholesterol exchange between red cell membranes and serum lipoproteins were studied by following the movement of tritiated cholesterol incorporated into erythrocytes .
	manualset3
148414	7	409793	5	NULL	NULL	0	NULL	tritiated cholesterol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of sickling on cholesterol exchange between red cell membranes and serum lipoproteins were studied by following the movement of tritiated cholesterol incorporated into erythrocytes .
	manualset3
148415	8	409793	5	NULL	NULL	0	NULL	erythrocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of sickling on cholesterol exchange between red cell membranes and serum lipoproteins were studied by following the movement of tritiated cholesterol incorporated into erythrocytes .
	manualset3
148416	1	409794	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of six compounds ( acetaminophen = AAP , isoniazid = INH , digoxin , malathion , paraquat and 2 , 4-dichlorophenoxy acetic acid = 2 , 4-D ) on cell cycle were investigated in HepG2 cells and the induction of apoptosis/necrosis was analyzed by a spectrum of flow cytometric assays in HepG2 , AAH-1 and YAC-1 cells .
	manualset3
148417	2	409794	5	NULL	NULL	0	NULL	six compounds	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of six compounds ( acetaminophen = AAP , isoniazid = INH , digoxin , malathion , paraquat and 2 , 4-dichlorophenoxy acetic acid = 2 , 4-D ) on cell cycle were investigated in HepG2 cells and the induction of apoptosis/necrosis was analyzed by a spectrum of flow cytometric assays in HepG2 , AAH-1 and YAC-1 cells .
	manualset3
148418	3	409794	5	NULL	NULL	0	NULL	acetaminophen = AAP	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of six compounds ( acetaminophen = AAP , isoniazid = INH , digoxin , malathion , paraquat and 2 , 4-dichlorophenoxy acetic acid = 2 , 4-D ) on cell cycle were investigated in HepG2 cells and the induction of apoptosis/necrosis was analyzed by a spectrum of flow cytometric assays in HepG2 , AAH-1 and YAC-1 cells .
	manualset3
148419	4	409794	5	NULL	NULL	0	NULL	isoniazid = INH	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of six compounds ( acetaminophen = AAP , isoniazid = INH , digoxin , malathion , paraquat and 2 , 4-dichlorophenoxy acetic acid = 2 , 4-D ) on cell cycle were investigated in HepG2 cells and the induction of apoptosis/necrosis was analyzed by a spectrum of flow cytometric assays in HepG2 , AAH-1 and YAC-1 cells .
	manualset3
148420	5	409794	5	NULL	NULL	0	NULL	digoxin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of six compounds ( acetaminophen = AAP , isoniazid = INH , digoxin , malathion , paraquat and 2 , 4-dichlorophenoxy acetic acid = 2 , 4-D ) on cell cycle were investigated in HepG2 cells and the induction of apoptosis/necrosis was analyzed by a spectrum of flow cytometric assays in HepG2 , AAH-1 and YAC-1 cells .
	manualset3
148421	6	409794	5	NULL	NULL	NULL	NULL	malathion 	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The effects of six compounds ( acetaminophen = AAP , isoniazid = INH , digoxin , malathion , paraquat and 2 , 4-dichlorophenoxy acetic acid = 2 , 4-D ) on cell cycle were investigated in HepG2 cells and the induction of apoptosis/necrosis was analyzed by a spectrum of flow cytometric assays in HepG2 , AAH-1 and YAC-1 cells .
	manualset3
148422	7	409794	5	NULL	NULL	0	NULL	paraquat 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of six compounds ( acetaminophen = AAP , isoniazid = INH , digoxin , malathion , paraquat and 2 , 4-dichlorophenoxy acetic acid = 2 , 4-D ) on cell cycle were investigated in HepG2 cells and the induction of apoptosis/necrosis was analyzed by a spectrum of flow cytometric assays in HepG2 , AAH-1 and YAC-1 cells .
	manualset3
148423	8	409794	5	NULL	NULL	0	NULL	2 , 4-dichlorophenoxy acetic acid = 2 , 4-D 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of six compounds ( acetaminophen = AAP , isoniazid = INH , digoxin , malathion , paraquat and 2 , 4-dichlorophenoxy acetic acid = 2 , 4-D ) on cell cycle were investigated in HepG2 cells and the induction of apoptosis/necrosis was analyzed by a spectrum of flow cytometric assays in HepG2 , AAH-1 and YAC-1 cells .
	manualset3
148424	9	409794	5	NULL	NULL	0	NULL	cell cycle 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of six compounds ( acetaminophen = AAP , isoniazid = INH , digoxin , malathion , paraquat and 2 , 4-dichlorophenoxy acetic acid = 2 , 4-D ) on cell cycle were investigated in HepG2 cells and the induction of apoptosis/necrosis was analyzed by a spectrum of flow cytometric assays in HepG2 , AAH-1 and YAC-1 cells .
	manualset3
148425	10	409794	5	NULL	NULL	0	NULL	HepG2 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of six compounds ( acetaminophen = AAP , isoniazid = INH , digoxin , malathion , paraquat and 2 , 4-dichlorophenoxy acetic acid = 2 , 4-D ) on cell cycle were investigated in HepG2 cells and the induction of apoptosis/necrosis was analyzed by a spectrum of flow cytometric assays in HepG2 , AAH-1 and YAC-1 cells .
	manualset3
148426	11	409794	5	NULL	NULL	0	NULL	induction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of six compounds ( acetaminophen = AAP , isoniazid = INH , digoxin , malathion , paraquat and 2 , 4-dichlorophenoxy acetic acid = 2 , 4-D ) on cell cycle were investigated in HepG2 cells and the induction of apoptosis/necrosis was analyzed by a spectrum of flow cytometric assays in HepG2 , AAH-1 and YAC-1 cells .
	manualset3
148427	12	409794	5	NULL	NULL	0	NULL	apoptosis/necrosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of six compounds ( acetaminophen = AAP , isoniazid = INH , digoxin , malathion , paraquat and 2 , 4-dichlorophenoxy acetic acid = 2 , 4-D ) on cell cycle were investigated in HepG2 cells and the induction of apoptosis/necrosis was analyzed by a spectrum of flow cytometric assays in HepG2 , AAH-1 and YAC-1 cells .
	manualset3
148428	13	409794	5	NULL	NULL	0	NULL	spectrum 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of six compounds ( acetaminophen = AAP , isoniazid = INH , digoxin , malathion , paraquat and 2 , 4-dichlorophenoxy acetic acid = 2 , 4-D ) on cell cycle were investigated in HepG2 cells and the induction of apoptosis/necrosis was analyzed by a spectrum of flow cytometric assays in HepG2 , AAH-1 and YAC-1 cells .
	manualset3
148429	14	409794	5	NULL	NULL	0	NULL	flow cytometric assays 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of six compounds ( acetaminophen = AAP , isoniazid = INH , digoxin , malathion , paraquat and 2 , 4-dichlorophenoxy acetic acid = 2 , 4-D ) on cell cycle were investigated in HepG2 cells and the induction of apoptosis/necrosis was analyzed by a spectrum of flow cytometric assays in HepG2 , AAH-1 and YAC-1 cells .
	manualset3
148430	15	409794	5	NULL	NULL	0	NULL	HepG2 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of six compounds ( acetaminophen = AAP , isoniazid = INH , digoxin , malathion , paraquat and 2 , 4-dichlorophenoxy acetic acid = 2 , 4-D ) on cell cycle were investigated in HepG2 cells and the induction of apoptosis/necrosis was analyzed by a spectrum of flow cytometric assays in HepG2 , AAH-1 and YAC-1 cells .
	manualset3
148431	16	409794	5	NULL	NULL	0	NULL	AAH-1 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of six compounds ( acetaminophen = AAP , isoniazid = INH , digoxin , malathion , paraquat and 2 , 4-dichlorophenoxy acetic acid = 2 , 4-D ) on cell cycle were investigated in HepG2 cells and the induction of apoptosis/necrosis was analyzed by a spectrum of flow cytometric assays in HepG2 , AAH-1 and YAC-1 cells .
	manualset3
148432	17	409794	5	NULL	NULL	0	NULL	YAC-1 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of six compounds ( acetaminophen = AAP , isoniazid = INH , digoxin , malathion , paraquat and 2 , 4-dichlorophenoxy acetic acid = 2 , 4-D ) on cell cycle were investigated in HepG2 cells and the induction of apoptosis/necrosis was analyzed by a spectrum of flow cytometric assays in HepG2 , AAH-1 and YAC-1 cells .
	manualset3
148433	1	409795	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of sodium dichloroacetate ( DCA ) on carbohydrate metabolism in conscious , 48-h-fasted dogs were examined using the hepatic A-V difference technique and a double isotope infusion technique ( 3H-glucose to measure glucose production and 14C-alanine to assess gluconeogenesis ) .
	manualset3
148434	2	409795	5	NULL	NULL	0	NULL	sodium dichloroacetate ( DCA )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of sodium dichloroacetate ( DCA ) on carbohydrate metabolism in conscious , 48-h-fasted dogs were examined using the hepatic A-V difference technique and a double isotope infusion technique ( 3H-glucose to measure glucose production and 14C-alanine to assess gluconeogenesis ) .
	manualset3
148435	3	409795	5	NULL	NULL	0	NULL	carbohydrate metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of sodium dichloroacetate ( DCA ) on carbohydrate metabolism in conscious , 48-h-fasted dogs were examined using the hepatic A-V difference technique and a double isotope infusion technique ( 3H-glucose to measure glucose production and 14C-alanine to assess gluconeogenesis ) .
	manualset3
148436	4	409795	5	NULL	NULL	0	NULL	conscious , 48-h-fasted dogs 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of sodium dichloroacetate ( DCA ) on carbohydrate metabolism in conscious , 48-h-fasted dogs were examined using the hepatic A-V difference technique and a double isotope infusion technique ( 3H-glucose to measure glucose production and 14C-alanine to assess gluconeogenesis ) .
	manualset3
148437	5	409795	5	NULL	NULL	0	NULL	hepatic A-V difference technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of sodium dichloroacetate ( DCA ) on carbohydrate metabolism in conscious , 48-h-fasted dogs were examined using the hepatic A-V difference technique and a double isotope infusion technique ( 3H-glucose to measure glucose production and 14C-alanine to assess gluconeogenesis ) .
	manualset3
148438	6	409795	5	NULL	NULL	0	NULL	double isotope infusion technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of sodium dichloroacetate ( DCA ) on carbohydrate metabolism in conscious , 48-h-fasted dogs were examined using the hepatic A-V difference technique and a double isotope infusion technique ( 3H-glucose to measure glucose production and 14C-alanine to assess gluconeogenesis ) .
	manualset3
148439	7	409795	5	NULL	NULL	0	NULL	3H-glucose	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of sodium dichloroacetate ( DCA ) on carbohydrate metabolism in conscious , 48-h-fasted dogs were examined using the hepatic A-V difference technique and a double isotope infusion technique ( 3H-glucose to measure glucose production and 14C-alanine to assess gluconeogenesis ) .
	manualset3
148440	8	409795	5	NULL	NULL	0	NULL	glucose production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of sodium dichloroacetate ( DCA ) on carbohydrate metabolism in conscious , 48-h-fasted dogs were examined using the hepatic A-V difference technique and a double isotope infusion technique ( 3H-glucose to measure glucose production and 14C-alanine to assess gluconeogenesis ) .
	manualset3
148441	9	409795	5	NULL	NULL	0	NULL	14C-alanine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of sodium dichloroacetate ( DCA ) on carbohydrate metabolism in conscious , 48-h-fasted dogs were examined using the hepatic A-V difference technique and a double isotope infusion technique ( 3H-glucose to measure glucose production and 14C-alanine to assess gluconeogenesis ) .
	manualset3
148442	10	409795	5	NULL	NULL	0	NULL	gluconeogenesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of sodium dichloroacetate ( DCA ) on carbohydrate metabolism in conscious , 48-h-fasted dogs were examined using the hepatic A-V difference technique and a double isotope infusion technique ( 3H-glucose to measure glucose production and 14C-alanine to assess gluconeogenesis ) .
	manualset3
148443	1	409796	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of substitution pattern on the pyridine ring , oxime substituent and 3-substituent were studied as a function of the MIC values .
	manualset3
148444	2	409796	5	NULL	NULL	0	NULL	substitution pattern	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of substitution pattern on the pyridine ring , oxime substituent and 3-substituent were studied as a function of the MIC values .
	manualset3
148445	3	409796	5	NULL	NULL	0	NULL	pyridine ring	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of substitution pattern on the pyridine ring , oxime substituent and 3-substituent were studied as a function of the MIC values .
	manualset3
148446	4	409796	5	NULL	NULL	0	NULL	oxime substituent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of substitution pattern on the pyridine ring , oxime substituent and 3-substituent were studied as a function of the MIC values .
	manualset3
148447	5	409796	5	NULL	NULL	0	NULL	3-substituent 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of substitution pattern on the pyridine ring , oxime substituent and 3-substituent were studied as a function of the MIC values .
	manualset3
148448	6	409796	5	NULL	NULL	0	NULL	function 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of substitution pattern on the pyridine ring , oxime substituent and 3-substituent were studied as a function of the MIC values .
	manualset3
148449	7	409796	5	NULL	NULL	0	NULL	 MIC values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of substitution pattern on the pyridine ring , oxime substituent and 3-substituent were studied as a function of the MIC values .
	manualset3
148450	1	409797	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the distance interaction between the irradiated and unirradiated corn plants in the conditions of water culture were investigated .
	manualset3
148451	2	409797	5	NULL	NULL	0	NULL	distance interaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the distance interaction between the irradiated and unirradiated corn plants in the conditions of water culture were investigated .
	manualset3
148452	3	409797	5	NULL	NULL	0	NULL	irradiated corn plants 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the distance interaction between the irradiated and unirradiated corn plants in the conditions of water culture were investigated .
	manualset3
148453	4	409797	5	NULL	NULL	0	NULL	unirradiated corn plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the distance interaction between the irradiated and unirradiated corn plants in the conditions of water culture were investigated .
	manualset3
148454	5	409797	5	NULL	NULL	0	NULL	conditions 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the distance interaction between the irradiated and unirradiated corn plants in the conditions of water culture were investigated .
	manualset3
148455	6	409797	5	NULL	NULL	0	NULL	water culture 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the distance interaction between the irradiated and unirradiated corn plants in the conditions of water culture were investigated .
	manualset3
148456	1	409798	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the eluted fractions on the uptake of urate and para-aminohippurate by isolated cortical tubules of rabbit kidney were investigated .
	manualset3
148457	2	409798	5	NULL	NULL	0	NULL	eluted fractions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the eluted fractions on the uptake of urate and para-aminohippurate by isolated cortical tubules of rabbit kidney were investigated .
	manualset3
148458	3	409798	5	NULL	NULL	0	NULL	uptake 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the eluted fractions on the uptake of urate and para-aminohippurate by isolated cortical tubules of rabbit kidney were investigated .
	manualset3
148459	4	409798	5	NULL	NULL	0	NULL	urate 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the eluted fractions on the uptake of urate and para-aminohippurate by isolated cortical tubules of rabbit kidney were investigated .
	manualset3
148460	5	409798	5	NULL	NULL	0	NULL	para-aminohippurate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the eluted fractions on the uptake of urate and para-aminohippurate by isolated cortical tubules of rabbit kidney were investigated .
	manualset3
148461	6	409798	5	NULL	NULL	0	NULL	isolated cortical tubules	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the eluted fractions on the uptake of urate and para-aminohippurate by isolated cortical tubules of rabbit kidney were investigated .
	manualset3
148462	7	409798	5	NULL	NULL	0	NULL	rabbit kidney	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the eluted fractions on the uptake of urate and para-aminohippurate by isolated cortical tubules of rabbit kidney were investigated .
	manualset3
148463	1	409799	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the strychnine-insensitive glycine receptor antagonists , cycloleucine and 7-chlorokynurenic acid , on the induction of long-term potentiation ( LTP ) in CA1 of rat hippocampal slices were examined .
	manualset3
148464	2	409799	5	NULL	NULL	NULL	NULL	strychnine-insensitive glycine receptor antagonists , cycloleucine	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The effects of the strychnine-insensitive glycine receptor antagonists , cycloleucine and 7-chlorokynurenic acid , on the induction of long-term potentiation ( LTP ) in CA1 of rat hippocampal slices were examined .
	manualset3
148465	3	409799	5	NULL	NULL	0	NULL	strychnine-insensitive glycine receptor antagonists , 7-chlorokynurenic acid	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the strychnine-insensitive glycine receptor antagonists , cycloleucine and 7-chlorokynurenic acid , on the induction of long-term potentiation ( LTP ) in CA1 of rat hippocampal slices were examined .
	manualset3
148466	4	409799	5	NULL	NULL	0	NULL	induction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the strychnine-insensitive glycine receptor antagonists , cycloleucine and 7-chlorokynurenic acid , on the induction of long-term potentiation ( LTP ) in CA1 of rat hippocampal slices were examined .
	manualset3
148467	5	409799	5	NULL	NULL	0	NULL	long-term potentiation ( LTP )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the strychnine-insensitive glycine receptor antagonists , cycloleucine and 7-chlorokynurenic acid , on the induction of long-term potentiation ( LTP ) in CA1 of rat hippocampal slices were examined .
	manualset3
148468	6	409799	5	NULL	NULL	0	NULL	CA1 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the strychnine-insensitive glycine receptor antagonists , cycloleucine and 7-chlorokynurenic acid , on the induction of long-term potentiation ( LTP ) in CA1 of rat hippocampal slices were examined .
	manualset3
148469	7	409799	5	NULL	NULL	0	NULL	rat hippocampal slices	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the strychnine-insensitive glycine receptor antagonists , cycloleucine and 7-chlorokynurenic acid , on the induction of long-term potentiation ( LTP ) in CA1 of rat hippocampal slices were examined .
	manualset3
148470	1	409800	5	NULL	NULL	0	NULL	strong cooperative effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A strong cooperative effect is obtained when few He atoms perturb the oxygen molecule .
	manualset3
148471	2	409800	5	NULL	NULL	0	NULL	He atoms 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	A strong cooperative effect is obtained when few He atoms perturb the oxygen molecule .
	manualset3
148472	3	409800	5	NULL	NULL	0	NULL	oxygen molecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A strong cooperative effect is obtained when few He atoms perturb the oxygen molecule .
	manualset3
148473	1	409801	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the synthetic non-psychoactive cannabinoid ( + ) - ( 3S , 4 S ) -7 - hydroxy-delta 6-tetrahydrocannabinol 1 , 1-dimethylheptyl ( HU-211 ) on the activity of the N-methyl-D-aspartate ( NMDA ) receptor/ion channel were examined .
	manualset3
148474	2	409801	5	NULL	NULL	0	NULL	 synthetic non-psychoactive cannabinoid ( + ) - ( 3S , 4 S ) -7 - hydroxy-delta 6-tetrahydrocannabinol 1 , 1-dimethylheptyl ( HU-211 ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the synthetic non-psychoactive cannabinoid ( + ) - ( 3S , 4 S ) -7 - hydroxy-delta 6-tetrahydrocannabinol 1 , 1-dimethylheptyl ( HU-211 ) on the activity of the N-methyl-D-aspartate ( NMDA ) receptor/ion channel were examined .
	manualset3
148475	3	409801	5	NULL	NULL	0	NULL	activity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the synthetic non-psychoactive cannabinoid ( + ) - ( 3S , 4 S ) -7 - hydroxy-delta 6-tetrahydrocannabinol 1 , 1-dimethylheptyl ( HU-211 ) on the activity of the N-methyl-D-aspartate ( NMDA ) receptor/ion channel were examined .
	manualset3
148476	4	409801	5	NULL	NULL	0	NULL	N-methyl-D-aspartate ( NMDA ) receptor/ion channel 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the synthetic non-psychoactive cannabinoid ( + ) - ( 3S , 4 S ) -7 - hydroxy-delta 6-tetrahydrocannabinol 1 , 1-dimethylheptyl ( HU-211 ) on the activity of the N-methyl-D-aspartate ( NMDA ) receptor/ion channel were examined .
	manualset3
148477	1	409802	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of these cytokines on HSF activity are related to variations of IL-6 and OSM secretion .
	manualset3
148478	2	409802	5	NULL	NULL	0	NULL	cytokines 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of these cytokines on HSF activity are related to variations of IL-6 and OSM secretion .
	manualset3
148479	3	409802	5	NULL	NULL	0	NULL	HSF activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of these cytokines on HSF activity are related to variations of IL-6 and OSM secretion .
	manualset3
148480	4	409802	5	NULL	NULL	0	NULL	variations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of these cytokines on HSF activity are related to variations of IL-6 and OSM secretion .
	manualset3
148481	5	409802	5	NULL	NULL	0	NULL	IL-6 secretion 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of these cytokines on HSF activity are related to variations of IL-6 and OSM secretion .
	manualset3
148482	6	409802	5	NULL	NULL	0	NULL	OSM secretion 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of these cytokines on HSF activity are related to variations of IL-6 and OSM secretion .
	manualset3
148483	1	409803	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of these limited perfusions were then compared with experiments in which the whole gut ( ALL ) was exposed to the nutrient .
	manualset3
148484	2	409803	5	NULL	NULL	0	NULL	limited perfusions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of these limited perfusions were then compared with experiments in which the whole gut ( ALL ) was exposed to the nutrient .
	manualset3
148485	3	409803	5	NULL	NULL	0	NULL	experiments 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of these limited perfusions were then compared with experiments in which the whole gut ( ALL ) was exposed to the nutrient .
	manualset3
148486	4	409803	5	NULL	NULL	0	NULL	whole gut ( ALL ) 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of these limited perfusions were then compared with experiments in which the whole gut ( ALL ) was exposed to the nutrient .
	manualset3
148487	5	409803	5	NULL	NULL	0	NULL	nutrient 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of these limited perfusions were then compared with experiments in which the whole gut ( ALL ) was exposed to the nutrient .
	manualset3
148488	1	409804	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of two common diluents ( microcrystalline cellulose and calcium phosphate dihydrate ) , two binding agents ( gelatin and methacrylic polymer ) , and spheronization on the micromeritic ( size , shape , density ) , flow , and packing properties of sodium diclofenac pellets were examined .
	manualset3
148489	2	409804	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of two common diluents ( microcrystalline cellulose and calcium phosphate dihydrate ) , two binding agents ( gelatin and methacrylic polymer ) , and spheronization on the micromeritic ( size , shape , density ) , flow , and packing properties of sodium diclofenac pellets were examined .
	manualset3
148490	3	409804	5	NULL	NULL	0	NULL	diluents 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of two common diluents ( microcrystalline cellulose and calcium phosphate dihydrate ) , two binding agents ( gelatin and methacrylic polymer ) , and spheronization on the micromeritic ( size , shape , density ) , flow , and packing properties of sodium diclofenac pellets were examined .
	manualset3
148491	4	409804	5	NULL	NULL	0	NULL	microcrystalline cellulose 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of two common diluents ( microcrystalline cellulose and calcium phosphate dihydrate ) , two binding agents ( gelatin and methacrylic polymer ) , and spheronization on the micromeritic ( size , shape , density ) , flow , and packing properties of sodium diclofenac pellets were examined .
	manualset3
148492	5	409804	5	NULL	NULL	0	NULL	calcium phosphate dihydrate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of two common diluents ( microcrystalline cellulose and calcium phosphate dihydrate ) , two binding agents ( gelatin and methacrylic polymer ) , and spheronization on the micromeritic ( size , shape , density ) , flow , and packing properties of sodium diclofenac pellets were examined .
	manualset3
148493	6	409804	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of two common diluents ( microcrystalline cellulose and calcium phosphate dihydrate ) , two binding agents ( gelatin and methacrylic polymer ) , and spheronization on the micromeritic ( size , shape , density ) , flow , and packing properties of sodium diclofenac pellets were examined .
	manualset3
148494	7	409804	5	NULL	NULL	NULL	NULL	binding agents	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The effects of two common diluents ( microcrystalline cellulose and calcium phosphate dihydrate ) , two binding agents ( gelatin and methacrylic polymer ) , and spheronization on the micromeritic ( size , shape , density ) , flow , and packing properties of sodium diclofenac pellets were examined .
	manualset3
148495	8	409804	5	NULL	NULL	0	NULL	gelatin 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of two common diluents ( microcrystalline cellulose and calcium phosphate dihydrate ) , two binding agents ( gelatin and methacrylic polymer ) , and spheronization on the micromeritic ( size , shape , density ) , flow , and packing properties of sodium diclofenac pellets were examined .
	manualset3
148496	9	409804	5	NULL	NULL	0	NULL	methacrylic polymer	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of two common diluents ( microcrystalline cellulose and calcium phosphate dihydrate ) , two binding agents ( gelatin and methacrylic polymer ) , and spheronization on the micromeritic ( size , shape , density ) , flow , and packing properties of sodium diclofenac pellets were examined .
	manualset3
148497	10	409804	5	NULL	NULL	0	NULL	spheronization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of two common diluents ( microcrystalline cellulose and calcium phosphate dihydrate ) , two binding agents ( gelatin and methacrylic polymer ) , and spheronization on the micromeritic ( size , shape , density ) , flow , and packing properties of sodium diclofenac pellets were examined .
	manualset3
148498	11	409804	5	NULL	NULL	0	NULL	size 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of two common diluents ( microcrystalline cellulose and calcium phosphate dihydrate ) , two binding agents ( gelatin and methacrylic polymer ) , and spheronization on the micromeritic ( size , shape , density ) , flow , and packing properties of sodium diclofenac pellets were examined .
	manualset3
148499	12	409804	5	NULL	NULL	0	NULL	shape 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of two common diluents ( microcrystalline cellulose and calcium phosphate dihydrate ) , two binding agents ( gelatin and methacrylic polymer ) , and spheronization on the micromeritic ( size , shape , density ) , flow , and packing properties of sodium diclofenac pellets were examined .
	manualset3
148500	13	409804	5	NULL	NULL	0	NULL	density 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of two common diluents ( microcrystalline cellulose and calcium phosphate dihydrate ) , two binding agents ( gelatin and methacrylic polymer ) , and spheronization on the micromeritic ( size , shape , density ) , flow , and packing properties of sodium diclofenac pellets were examined .
	manualset3
148501	14	409804	5	NULL	NULL	0	NULL	flow 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of two common diluents ( microcrystalline cellulose and calcium phosphate dihydrate ) , two binding agents ( gelatin and methacrylic polymer ) , and spheronization on the micromeritic ( size , shape , density ) , flow , and packing properties of sodium diclofenac pellets were examined .
	manualset3
148502	15	409804	5	NULL	NULL	0	NULL	packing properties 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of two common diluents ( microcrystalline cellulose and calcium phosphate dihydrate ) , two binding agents ( gelatin and methacrylic polymer ) , and spheronization on the micromeritic ( size , shape , density ) , flow , and packing properties of sodium diclofenac pellets were examined .
	manualset3
148503	16	409804	5	NULL	NULL	0	NULL	sodium diclofenac pellets 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of two common diluents ( microcrystalline cellulose and calcium phosphate dihydrate ) , two binding agents ( gelatin and methacrylic polymer ) , and spheronization on the micromeritic ( size , shape , density ) , flow , and packing properties of sodium diclofenac pellets were examined .
	manualset3
148504	1	409805	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of various mitochondrial coenzymes and metabolities on the activities of 3-oxoacyl-CoA thiolase ( EC 2.3.1.16 ) and acetoacetyl-CoA thiolase ( EC 2.3.1.9 ) from pig heart were investigated with the aim of elucidating the possible regulation of these two enzymes .
	manualset3
148505	2	409805	5	NULL	NULL	0	NULL	mitochondrial coenzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of various mitochondrial coenzymes and metabolities on the activities of 3-oxoacyl-CoA thiolase ( EC 2.3.1.16 ) and acetoacetyl-CoA thiolase ( EC 2.3.1.9 ) from pig heart were investigated with the aim of elucidating the possible regulation of these two enzymes .
	manualset3
148506	3	409805	5	NULL	NULL	0	NULL	metabolities 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of various mitochondrial coenzymes and metabolities on the activities of 3-oxoacyl-CoA thiolase ( EC 2.3.1.16 ) and acetoacetyl-CoA thiolase ( EC 2.3.1.9 ) from pig heart were investigated with the aim of elucidating the possible regulation of these two enzymes .
	manualset3
148507	4	409805	5	NULL	NULL	0	NULL	activities 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of various mitochondrial coenzymes and metabolities on the activities of 3-oxoacyl-CoA thiolase ( EC 2.3.1.16 ) and acetoacetyl-CoA thiolase ( EC 2.3.1.9 ) from pig heart were investigated with the aim of elucidating the possible regulation of these two enzymes .
	manualset3
148508	5	409805	5	NULL	NULL	0	NULL	3-oxoacyl-CoA thiolase ( EC 2.3.1.16 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of various mitochondrial coenzymes and metabolities on the activities of 3-oxoacyl-CoA thiolase ( EC 2.3.1.16 ) and acetoacetyl-CoA thiolase ( EC 2.3.1.9 ) from pig heart were investigated with the aim of elucidating the possible regulation of these two enzymes .
	manualset3
148509	6	409805	5	NULL	NULL	0	NULL	acetoacetyl-CoA thiolase ( EC 2.3.1.9 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of various mitochondrial coenzymes and metabolities on the activities of 3-oxoacyl-CoA thiolase ( EC 2.3.1.16 ) and acetoacetyl-CoA thiolase ( EC 2.3.1.9 ) from pig heart were investigated with the aim of elucidating the possible regulation of these two enzymes .
	manualset3
148510	7	409805	5	NULL	NULL	0	NULL	pig heart	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of various mitochondrial coenzymes and metabolities on the activities of 3-oxoacyl-CoA thiolase ( EC 2.3.1.16 ) and acetoacetyl-CoA thiolase ( EC 2.3.1.9 ) from pig heart were investigated with the aim of elucidating the possible regulation of these two enzymes .
	manualset3
148511	8	409805	5	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of various mitochondrial coenzymes and metabolities on the activities of 3-oxoacyl-CoA thiolase ( EC 2.3.1.16 ) and acetoacetyl-CoA thiolase ( EC 2.3.1.9 ) from pig heart were investigated with the aim of elucidating the possible regulation of these two enzymes .
	manualset3
148512	9	409805	5	NULL	NULL	0	NULL	regulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of various mitochondrial coenzymes and metabolities on the activities of 3-oxoacyl-CoA thiolase ( EC 2.3.1.16 ) and acetoacetyl-CoA thiolase ( EC 2.3.1.9 ) from pig heart were investigated with the aim of elucidating the possible regulation of these two enzymes .
	manualset3
148513	10	409805	5	NULL	NULL	0	NULL	two 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of various mitochondrial coenzymes and metabolities on the activities of 3-oxoacyl-CoA thiolase ( EC 2.3.1.16 ) and acetoacetyl-CoA thiolase ( EC 2.3.1.9 ) from pig heart were investigated with the aim of elucidating the possible regulation of these two enzymes .
	manualset3
148514	11	409805	5	NULL	NULL	0	NULL	enzymes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of various mitochondrial coenzymes and metabolities on the activities of 3-oxoacyl-CoA thiolase ( EC 2.3.1.16 ) and acetoacetyl-CoA thiolase ( EC 2.3.1.9 ) from pig heart were investigated with the aim of elucidating the possible regulation of these two enzymes .
	manualset3
148515	1	409806	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of various morphine-N-allyl-normorphine ratios on behavior .
	manualset3
148516	2	409806	5	NULL	NULL	0	NULL	morphine-N-allyl-normorphine ratios	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of various morphine-N-allyl-normorphine ratios on behavior .
	manualset3
148517	3	409806	5	NULL	NULL	0	NULL	behavior 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of various morphine-N-allyl-normorphine ratios on behavior .
	manualset3
148518	1	409807	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects on serum calcium , potassium and uric acid were in accordance with previous reports .
	manualset3
148519	2	409807	5	NULL	NULL	0	NULL	serum calcium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects on serum calcium , potassium and uric acid were in accordance with previous reports .
	manualset3
148520	3	409807	5	NULL	NULL	0	NULL	potassium 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects on serum calcium , potassium and uric acid were in accordance with previous reports .
	manualset3
148521	4	409807	5	NULL	NULL	0	NULL	uric acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects on serum calcium , potassium and uric acid were in accordance with previous reports .
	manualset3
148522	5	409807	5	NULL	NULL	0	NULL	previous reports	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects on serum calcium , potassium and uric acid were in accordance with previous reports .
	manualset3
148523	1	409808	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects were not as pronounced as for CYP24 .
	manualset3
148524	2	409808	5	NULL	NULL	0	NULL	CYP24 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects were not as pronounced as for CYP24 .
	manualset3
148525	1	409809	5	NULL	NULL	0	NULL	structural perspective 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A structural and functional perspective into the mechanism of Ca2 + - sensitizers that target the cardiac troponin complex .
	manualset3
148526	2	409809	5	NULL	NULL	0	NULL	functional perspective 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A structural and functional perspective into the mechanism of Ca2 + - sensitizers that target the cardiac troponin complex .
	manualset3
148527	3	409809	5	NULL	NULL	0	NULL	mechanism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A structural and functional perspective into the mechanism of Ca2 + - sensitizers that target the cardiac troponin complex .
	manualset3
148528	4	409809	5	NULL	NULL	0	NULL	Ca2 + - sensitizers	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A structural and functional perspective into the mechanism of Ca2 + - sensitizers that target the cardiac troponin complex .
	manualset3
148529	5	409809	5	NULL	NULL	0	NULL	cardiac troponin complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A structural and functional perspective into the mechanism of Ca2 + - sensitizers that target the cardiac troponin complex .
	manualset3
148530	1	409810	5	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects were not correlated with the presence of classical opiate receptors on the cells .
	manualset3
148531	2	409810	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects were not correlated with the presence of classical opiate receptors on the cells .
	manualset3
148532	3	409810	5	NULL	NULL	0	NULL	classical opiate receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects were not correlated with the presence of classical opiate receptors on the cells .
	manualset3
148533	4	409810	5	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects were not correlated with the presence of classical opiate receptors on the cells .
	manualset3
148534	1	409811	5	NULL	NULL	0	NULL	efficacy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy and economical viability of vaccination against respiratory disease in calves remains unclear .
	manualset3
148535	2	409811	5	NULL	NULL	0	NULL	economical viability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy and economical viability of vaccination against respiratory disease in calves remains unclear .
	manualset3
148536	3	409811	5	NULL	NULL	0	NULL	vaccination 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy and economical viability of vaccination against respiratory disease in calves remains unclear .
	manualset3
148537	4	409811	5	NULL	NULL	0	NULL	respiratory disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy and economical viability of vaccination against respiratory disease in calves remains unclear .
	manualset3
148538	5	409811	5	NULL	NULL	0	NULL	calves 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy and economical viability of vaccination against respiratory disease in calves remains unclear .
	manualset3
148539	1	409812	5	NULL	NULL	0	NULL	efficacy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy and safety of ofloxacin in the treatment of upper and lower urinary tract infections were studied with the drug use according to 4 regimens by comparison with nitrofurantoin in the treatment of lower urinary tract infections and trimethoprim/sulfamethoxazole in the treatment of upper urinary tract infections .
	manualset3
148540	2	409812	5	NULL	NULL	0	NULL	safety 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy and safety of ofloxacin in the treatment of upper and lower urinary tract infections were studied with the drug use according to 4 regimens by comparison with nitrofurantoin in the treatment of lower urinary tract infections and trimethoprim/sulfamethoxazole in the treatment of upper urinary tract infections .
	manualset3
148541	3	409812	5	NULL	NULL	0	NULL	ofloxacin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy and safety of ofloxacin in the treatment of upper and lower urinary tract infections were studied with the drug use according to 4 regimens by comparison with nitrofurantoin in the treatment of lower urinary tract infections and trimethoprim/sulfamethoxazole in the treatment of upper urinary tract infections .
	manualset3
148542	4	409812	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy and safety of ofloxacin in the treatment of upper and lower urinary tract infections were studied with the drug use according to 4 regimens by comparison with nitrofurantoin in the treatment of lower urinary tract infections and trimethoprim/sulfamethoxazole in the treatment of upper urinary tract infections .
	manualset3
148543	5	409812	5	NULL	NULL	0	NULL	upper and lower urinary tract infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy and safety of ofloxacin in the treatment of upper and lower urinary tract infections were studied with the drug use according to 4 regimens by comparison with nitrofurantoin in the treatment of lower urinary tract infections and trimethoprim/sulfamethoxazole in the treatment of upper urinary tract infections .
	manualset3
148544	6	409812	5	NULL	NULL	0	NULL	drug use	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy and safety of ofloxacin in the treatment of upper and lower urinary tract infections were studied with the drug use according to 4 regimens by comparison with nitrofurantoin in the treatment of lower urinary tract infections and trimethoprim/sulfamethoxazole in the treatment of upper urinary tract infections .
	manualset3
148545	7	409812	5	NULL	NULL	0	NULL	4 regimens	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy and safety of ofloxacin in the treatment of upper and lower urinary tract infections were studied with the drug use according to 4 regimens by comparison with nitrofurantoin in the treatment of lower urinary tract infections and trimethoprim/sulfamethoxazole in the treatment of upper urinary tract infections .
	manualset3
148546	8	409812	5	NULL	NULL	0	NULL	comparison 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy and safety of ofloxacin in the treatment of upper and lower urinary tract infections were studied with the drug use according to 4 regimens by comparison with nitrofurantoin in the treatment of lower urinary tract infections and trimethoprim/sulfamethoxazole in the treatment of upper urinary tract infections .
	manualset3
148547	9	409812	5	NULL	NULL	0	NULL	nitrofurantoin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy and safety of ofloxacin in the treatment of upper and lower urinary tract infections were studied with the drug use according to 4 regimens by comparison with nitrofurantoin in the treatment of lower urinary tract infections and trimethoprim/sulfamethoxazole in the treatment of upper urinary tract infections .
	manualset3
148548	10	409812	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy and safety of ofloxacin in the treatment of upper and lower urinary tract infections were studied with the drug use according to 4 regimens by comparison with nitrofurantoin in the treatment of lower urinary tract infections and trimethoprim/sulfamethoxazole in the treatment of upper urinary tract infections .
	manualset3
148549	11	409812	5	NULL	NULL	0	NULL	lower urinary tract infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy and safety of ofloxacin in the treatment of upper and lower urinary tract infections were studied with the drug use according to 4 regimens by comparison with nitrofurantoin in the treatment of lower urinary tract infections and trimethoprim/sulfamethoxazole in the treatment of upper urinary tract infections .
	manualset3
148550	12	409812	5	NULL	NULL	0	NULL	trimethoprim/sulfamethoxazole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy and safety of ofloxacin in the treatment of upper and lower urinary tract infections were studied with the drug use according to 4 regimens by comparison with nitrofurantoin in the treatment of lower urinary tract infections and trimethoprim/sulfamethoxazole in the treatment of upper urinary tract infections .
	manualset3
148551	13	409812	5	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy and safety of ofloxacin in the treatment of upper and lower urinary tract infections were studied with the drug use according to 4 regimens by comparison with nitrofurantoin in the treatment of lower urinary tract infections and trimethoprim/sulfamethoxazole in the treatment of upper urinary tract infections .
	manualset3
148552	14	409812	5	NULL	NULL	0	NULL	upper urinary tract infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy and safety of ofloxacin in the treatment of upper and lower urinary tract infections were studied with the drug use according to 4 regimens by comparison with nitrofurantoin in the treatment of lower urinary tract infections and trimethoprim/sulfamethoxazole in the treatment of upper urinary tract infections .
	manualset3
148553	1	409813	5	NULL	NULL	0	NULL	efficacy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy and safety of recombinant human erythropoietin ( rhEPO ) were tested when given subcutaneously ( s.c. ) in an escalating dose of 2000-10 , 000 units ( U ) daily in 60 patients with cancer-related anemia ( CRA ) .
	manualset3
148554	2	409813	5	NULL	NULL	0	NULL	safety 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy and safety of recombinant human erythropoietin ( rhEPO ) were tested when given subcutaneously ( s.c. ) in an escalating dose of 2000-10 , 000 units ( U ) daily in 60 patients with cancer-related anemia ( CRA ) .
	manualset3
148555	3	409813	5	NULL	NULL	0	NULL	recombinant human erythropoietin ( rhEPO )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy and safety of recombinant human erythropoietin ( rhEPO ) were tested when given subcutaneously ( s.c. ) in an escalating dose of 2000-10 , 000 units ( U ) daily in 60 patients with cancer-related anemia ( CRA ) .
	manualset3
148556	4	409813	5	NULL	NULL	0	NULL	escalating dose 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy and safety of recombinant human erythropoietin ( rhEPO ) were tested when given subcutaneously ( s.c. ) in an escalating dose of 2000-10 , 000 units ( U ) daily in 60 patients with cancer-related anemia ( CRA ) .
	manualset3
148557	5	409813	5	NULL	NULL	0	NULL	2000-10 , 000 units ( U ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy and safety of recombinant human erythropoietin ( rhEPO ) were tested when given subcutaneously ( s.c. ) in an escalating dose of 2000-10 , 000 units ( U ) daily in 60 patients with cancer-related anemia ( CRA ) .
	manualset3
148558	6	409813	5	NULL	NULL	0	NULL	60 patients	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy and safety of recombinant human erythropoietin ( rhEPO ) were tested when given subcutaneously ( s.c. ) in an escalating dose of 2000-10 , 000 units ( U ) daily in 60 patients with cancer-related anemia ( CRA ) .
	manualset3
148559	7	409813	5	NULL	NULL	0	NULL	cancer-related anemia ( CRA )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy and safety of recombinant human erythropoietin ( rhEPO ) were tested when given subcutaneously ( s.c. ) in an escalating dose of 2000-10 , 000 units ( U ) daily in 60 patients with cancer-related anemia ( CRA ) .
	manualset3
148560	1	409814	5	NULL	NULL	0	NULL	efficacy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of Pyrithione , Pimafucin and Amphotericin B was compared in experimental adiaspiromycosis , Pyrithione showed also in vivo the best therapeutic effect .
	manualset3
148561	2	409814	5	NULL	NULL	0	NULL	Pyrithione 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of Pyrithione , Pimafucin and Amphotericin B was compared in experimental adiaspiromycosis , Pyrithione showed also in vivo the best therapeutic effect .
	manualset3
148562	3	409814	5	NULL	NULL	0	NULL	Pimafucin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of Pyrithione , Pimafucin and Amphotericin B was compared in experimental adiaspiromycosis , Pyrithione showed also in vivo the best therapeutic effect .
	manualset3
148563	4	409814	5	NULL	NULL	0	NULL	Amphotericin B	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of Pyrithione , Pimafucin and Amphotericin B was compared in experimental adiaspiromycosis , Pyrithione showed also in vivo the best therapeutic effect .
	manualset3
148564	5	409814	5	NULL	NULL	0	NULL	experimental adiaspiromycosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of Pyrithione , Pimafucin and Amphotericin B was compared in experimental adiaspiromycosis , Pyrithione showed also in vivo the best therapeutic effect .
	manualset3
148565	6	409814	5	NULL	NULL	0	NULL	Pyrithione 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of Pyrithione , Pimafucin and Amphotericin B was compared in experimental adiaspiromycosis , Pyrithione showed also in vivo the best therapeutic effect .
	manualset3
148566	7	409814	5	NULL	NULL	0	NULL	therapeutic effect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of Pyrithione , Pimafucin and Amphotericin B was compared in experimental adiaspiromycosis , Pyrithione showed also in vivo the best therapeutic effect .
	manualset3
148567	1	409815	5	NULL	NULL	0	NULL	efficacy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of acetylsalicylic acid ( ASA , aspirin ) and clopidogrel in decreasing the risk of adverse events in coronary heart disease patients has been well established in the past 20 years .
	manualset3
148568	2	409815	5	NULL	NULL	0	NULL	acetylsalicylic acid ( ASA , aspirin )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of acetylsalicylic acid ( ASA , aspirin ) and clopidogrel in decreasing the risk of adverse events in coronary heart disease patients has been well established in the past 20 years .
	manualset3
148569	3	409815	5	NULL	NULL	0	NULL	clopidogrel 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of acetylsalicylic acid ( ASA , aspirin ) and clopidogrel in decreasing the risk of adverse events in coronary heart disease patients has been well established in the past 20 years .
	manualset3
148570	4	409815	5	NULL	NULL	0	NULL	risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of acetylsalicylic acid ( ASA , aspirin ) and clopidogrel in decreasing the risk of adverse events in coronary heart disease patients has been well established in the past 20 years .
	manualset3
148571	5	409815	5	NULL	NULL	0	NULL	adverse events 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of acetylsalicylic acid ( ASA , aspirin ) and clopidogrel in decreasing the risk of adverse events in coronary heart disease patients has been well established in the past 20 years .
	manualset3
148572	6	409815	5	NULL	NULL	0	NULL	coronary heart disease patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of acetylsalicylic acid ( ASA , aspirin ) and clopidogrel in decreasing the risk of adverse events in coronary heart disease patients has been well established in the past 20 years .
	manualset3
148573	7	409815	5	NULL	NULL	0	NULL	20 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of acetylsalicylic acid ( ASA , aspirin ) and clopidogrel in decreasing the risk of adverse events in coronary heart disease patients has been well established in the past 20 years .
	manualset3
148574	1	409816	5	NULL	NULL	0	NULL	efficacy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of adenovirus ( ADV ) - mediated gene therapy to treat brain tumors was tested in a syngeneic glioma model .
	manualset3
148575	2	409816	5	NULL	NULL	0	NULL	adenovirus ( ADV ) - mediated gene therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of adenovirus ( ADV ) - mediated gene therapy to treat brain tumors was tested in a syngeneic glioma model .
	manualset3
148576	3	409816	5	NULL	NULL	0	NULL	brain tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of adenovirus ( ADV ) - mediated gene therapy to treat brain tumors was tested in a syngeneic glioma model .
	manualset3
148577	4	409816	5	NULL	NULL	0	NULL	syngeneic glioma model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of adenovirus ( ADV ) - mediated gene therapy to treat brain tumors was tested in a syngeneic glioma model .
	manualset3
148578	1	409817	5	NULL	NULL	0	NULL	efficacy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of the CPV component was studied both by monitoring antibody titers for more than a year and by challenge exposure of some dogs to virulent CPV .
	manualset3
148579	2	409817	5	NULL	NULL	0	NULL	CPV component	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of the CPV component was studied both by monitoring antibody titers for more than a year and by challenge exposure of some dogs to virulent CPV .
	manualset3
148580	3	409817	5	NULL	NULL	0	NULL	antibody titers	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of the CPV component was studied both by monitoring antibody titers for more than a year and by challenge exposure of some dogs to virulent CPV .
	manualset3
148581	4	409817	5	NULL	NULL	0	NULL	year 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of the CPV component was studied both by monitoring antibody titers for more than a year and by challenge exposure of some dogs to virulent CPV .
	manualset3
148582	5	409817	5	NULL	NULL	0	NULL	challenge exposure 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of the CPV component was studied both by monitoring antibody titers for more than a year and by challenge exposure of some dogs to virulent CPV .
	manualset3
148583	6	409817	5	NULL	NULL	0	NULL	dogs 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of the CPV component was studied both by monitoring antibody titers for more than a year and by challenge exposure of some dogs to virulent CPV .
	manualset3
148584	7	409817	5	NULL	NULL	0	NULL	virulent CPV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of the CPV component was studied both by monitoring antibody titers for more than a year and by challenge exposure of some dogs to virulent CPV .
	manualset3
148585	1	409818	5	NULL	NULL	0	NULL	efficacy 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of the embedded zero-tree wavelet compression algorithm is examined with respect to some important analysis parameters ( the length of the analysis segment and wavelet type ) and measurement conditions ( muscle type and contraction type ) .
	manualset3
148586	2	409818	5	NULL	NULL	0	NULL	embedded zero-tree wavelet compression algorithm	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of the embedded zero-tree wavelet compression algorithm is examined with respect to some important analysis parameters ( the length of the analysis segment and wavelet type ) and measurement conditions ( muscle type and contraction type ) .
	manualset3
148587	3	409818	5	NULL	NULL	0	NULL	analysis parameters	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of the embedded zero-tree wavelet compression algorithm is examined with respect to some important analysis parameters ( the length of the analysis segment and wavelet type ) and measurement conditions ( muscle type and contraction type ) .
	manualset3
148588	4	409818	5	NULL	NULL	0	NULL	length 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of the embedded zero-tree wavelet compression algorithm is examined with respect to some important analysis parameters ( the length of the analysis segment and wavelet type ) and measurement conditions ( muscle type and contraction type ) .
	manualset3
148589	5	409818	5	NULL	NULL	0	NULL	analysis segment 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of the embedded zero-tree wavelet compression algorithm is examined with respect to some important analysis parameters ( the length of the analysis segment and wavelet type ) and measurement conditions ( muscle type and contraction type ) .
	manualset3
148590	6	409818	5	NULL	NULL	0	NULL	wavelet type	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of the embedded zero-tree wavelet compression algorithm is examined with respect to some important analysis parameters ( the length of the analysis segment and wavelet type ) and measurement conditions ( muscle type and contraction type ) .
	manualset3
148591	7	409818	5	NULL	NULL	0	NULL	measurement conditions 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of the embedded zero-tree wavelet compression algorithm is examined with respect to some important analysis parameters ( the length of the analysis segment and wavelet type ) and measurement conditions ( muscle type and contraction type ) .
	manualset3
148592	8	409818	5	NULL	NULL	0	NULL	muscle type	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of the embedded zero-tree wavelet compression algorithm is examined with respect to some important analysis parameters ( the length of the analysis segment and wavelet type ) and measurement conditions ( muscle type and contraction type ) .
	manualset3
148593	9	409818	5	NULL	NULL	0	NULL	contraction type	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of the embedded zero-tree wavelet compression algorithm is examined with respect to some important analysis parameters ( the length of the analysis segment and wavelet type ) and measurement conditions ( muscle type and contraction type ) .
	manualset3
148594	1	409819	5	NULL	NULL	0	NULL	efficacy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy persisted throughout the repeated treatment period of 14 days without any evidence for the development of tolerance .
	manualset3
148595	2	409819	5	NULL	NULL	0	NULL	repeated treatment period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy persisted throughout the repeated treatment period of 14 days without any evidence for the development of tolerance .
	manualset3
148596	3	409819	5	NULL	NULL	0	NULL	14 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy persisted throughout the repeated treatment period of 14 days without any evidence for the development of tolerance .
	manualset3
148597	4	409819	5	NULL	NULL	0	NULL	evidence 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy persisted throughout the repeated treatment period of 14 days without any evidence for the development of tolerance .
	manualset3
148598	1	409820	5	NULL	NULL	0	NULL	family of oxidized phospholipids	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A structurally conserved family of oxidized phospholipids that serve as endogenous high-affinity ligands for the macrophage scavenger receptor CD36 ( oxPC ( CD36 ) ) was recently identified .
	manualset3
148599	2	409820	5	NULL	NULL	0	NULL	endogenous high-affinity ligands	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A structurally conserved family of oxidized phospholipids that serve as endogenous high-affinity ligands for the macrophage scavenger receptor CD36 ( oxPC ( CD36 ) ) was recently identified .
	manualset3
148600	3	409820	5	NULL	NULL	0	NULL	macrophage scavenger receptor CD36 ( oxPC ( CD36 ) ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A structurally conserved family of oxidized phospholipids that serve as endogenous high-affinity ligands for the macrophage scavenger receptor CD36 ( oxPC ( CD36 ) ) was recently identified .
	manualset3
148601	1	409821	5	NULL	NULL	0	NULL	efficiency 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficiency of cross-linking is dependent on the wavelength of the exciting radiation , on the nucleotide composition of the nucleic acid , and on the total photon flux .
	manualset3
148602	2	409821	5	NULL	NULL	0	NULL	wavelength 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficiency of cross-linking is dependent on the wavelength of the exciting radiation , on the nucleotide composition of the nucleic acid , and on the total photon flux .
	manualset3
148603	3	409821	5	NULL	NULL	0	NULL	exciting radiation	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficiency of cross-linking is dependent on the wavelength of the exciting radiation , on the nucleotide composition of the nucleic acid , and on the total photon flux .
	manualset3
148604	4	409821	5	NULL	NULL	0	NULL	nucleotide composition	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficiency of cross-linking is dependent on the wavelength of the exciting radiation , on the nucleotide composition of the nucleic acid , and on the total photon flux .
	manualset3
148605	5	409821	5	NULL	NULL	0	NULL	nucleic acid 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficiency of cross-linking is dependent on the wavelength of the exciting radiation , on the nucleotide composition of the nucleic acid , and on the total photon flux .
	manualset3
148606	6	409821	5	NULL	NULL	0	NULL	total photon flux	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficiency of cross-linking is dependent on the wavelength of the exciting radiation , on the nucleotide composition of the nucleic acid , and on the total photon flux .
	manualset3
148607	1	409822	5	NULL	NULL	0	NULL	efficiency 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficiency of the acoustophoretic washing principle was demonstrated by an unspecific phage cross contamination level of only 10 ( -6 ) of that in the input bead/phage mixture .
	manualset3
148608	2	409822	5	NULL	NULL	0	NULL	acoustophoretic washing principle 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficiency of the acoustophoretic washing principle was demonstrated by an unspecific phage cross contamination level of only 10 ( -6 ) of that in the input bead/phage mixture .
	manualset3
148609	3	409822	5	NULL	NULL	0	NULL	unspecific phage cross contamination level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficiency of the acoustophoretic washing principle was demonstrated by an unspecific phage cross contamination level of only 10 ( -6 ) of that in the input bead/phage mixture .
	manualset3
148610	4	409822	5	NULL	NULL	0	NULL	10 ( -6 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficiency of the acoustophoretic washing principle was demonstrated by an unspecific phage cross contamination level of only 10 ( -6 ) of that in the input bead/phage mixture .
	manualset3
148611	5	409822	5	NULL	NULL	0	NULL	input bead/phage mixture	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficiency of the acoustophoretic washing principle was demonstrated by an unspecific phage cross contamination level of only 10 ( -6 ) of that in the input bead/phage mixture .
	manualset3
148612	1	409823	5	NULL	NULL	0	NULL	efflux 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The efflux of this amine declined subsequently despite the continued presence of amphetamine in the CSF .
	manualset3
148613	2	409823	5	NULL	NULL	0	NULL	amine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The efflux of this amine declined subsequently despite the continued presence of amphetamine in the CSF .
	manualset3
148614	3	409823	5	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The efflux of this amine declined subsequently despite the continued presence of amphetamine in the CSF .
	manualset3
148615	4	409823	5	NULL	NULL	0	NULL	amphetamine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The efflux of this amine declined subsequently despite the continued presence of amphetamine in the CSF .
	manualset3
148616	5	409823	5	NULL	NULL	0	NULL	CSF 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The efflux of this amine declined subsequently despite the continued presence of amphetamine in the CSF .
	manualset3
148617	1	409824	5	NULL	NULL	0	NULL	effort 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effort has the support from 7 international pharmaceutical companies to participate .
	manualset3
148618	2	409824	5	NULL	NULL	0	NULL	support 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effort has the support from 7 international pharmaceutical companies to participate .
	manualset3
148619	3	409824	5	NULL	NULL	0	NULL	7	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The effort has the support from 7 international pharmaceutical companies to participate .
	manualset3
148620	4	409824	5	NULL	NULL	0	NULL	international pharmaceutical companies	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The effort has the support from 7 international pharmaceutical companies to participate .
	manualset3
148621	1	409825	5	NULL	NULL	0	NULL	elastic behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The elastic and anelastic behavior of elastomeric impression materials .
	manualset3
148622	2	409825	5	NULL	NULL	0	NULL	anelastic behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The elastic and anelastic behavior of elastomeric impression materials .
	manualset3
148623	3	409825	5	NULL	NULL	0	NULL	elastomeric impression materials	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The elastic and anelastic behavior of elastomeric impression materials .
	manualset3
148624	1	409826	5	NULL	NULL	0	NULL	eldest autopsied case ( a 23-year-old man ) 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The eldest autopsied case ( a 23-year-old man ) of infantile form of cystinosis with uremia and myxoedema was reported .
	manualset3
148625	2	409826	5	NULL	NULL	0	NULL	infantile form of cystinosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The eldest autopsied case ( a 23-year-old man ) of infantile form of cystinosis with uremia and myxoedema was reported .
	manualset3
148626	3	409826	5	NULL	NULL	0	NULL	uremia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The eldest autopsied case ( a 23-year-old man ) of infantile form of cystinosis with uremia and myxoedema was reported .
	manualset3
148627	4	409826	5	NULL	NULL	0	NULL	myxoedema 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The eldest autopsied case ( a 23-year-old man ) of infantile form of cystinosis with uremia and myxoedema was reported .
	manualset3
148628	1	409827	5	NULL	NULL	0	NULL	electric fields	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The electric fields induced by Labmag were half the size of those induced by MagPro at identical stimulus intensities .
	manualset3
148629	2	409827	5	NULL	NULL	0	NULL	Labmag 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The electric fields induced by Labmag were half the size of those induced by MagPro at identical stimulus intensities .
	manualset3
148630	3	409827	5	NULL	NULL	0	NULL	half the size	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The electric fields induced by Labmag were half the size of those induced by MagPro at identical stimulus intensities .
	manualset3
148631	4	409827	5	NULL	NULL	0	NULL	MagPro	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The electric fields induced by Labmag were half the size of those induced by MagPro at identical stimulus intensities .
	manualset3
148632	5	409827	5	NULL	NULL	0	NULL	stimulus intensities 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The electric fields induced by Labmag were half the size of those induced by MagPro at identical stimulus intensities .
	manualset3
148633	1	409828	5	NULL	NULL	NULL	NULL	electrocorticogram 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The electrocorticogram of both hemispheres , the neck electromyogram , the electrooculogram and electrocardiogram were recorded with implanted electrodes .
	manualset3
148634	2	409828	5	NULL	NULL	0	NULL	hemispheres 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrocorticogram of both hemispheres , the neck electromyogram , the electrooculogram and electrocardiogram were recorded with implanted electrodes .
	manualset3
148635	3	409828	5	NULL	NULL	0	NULL	neck electromyogram	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrocorticogram of both hemispheres , the neck electromyogram , the electrooculogram and electrocardiogram were recorded with implanted electrodes .
	manualset3
148636	4	409828	5	NULL	NULL	NULL	NULL	electrooculogram 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The electrocorticogram of both hemispheres , the neck electromyogram , the electrooculogram and electrocardiogram were recorded with implanted electrodes .
	manualset3
148637	5	409828	5	NULL	NULL	0	NULL	electrocardiogram 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrocorticogram of both hemispheres , the neck electromyogram , the electrooculogram and electrocardiogram were recorded with implanted electrodes .
	manualset3
148638	6	409828	5	NULL	NULL	0	NULL	implanted electrodes	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrocorticogram of both hemispheres , the neck electromyogram , the electrooculogram and electrocardiogram were recorded with implanted electrodes .
	manualset3
148639	1	409829	5	NULL	NULL	0	NULL	electrode 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrode exhibited a Nernstian response for strontium ion over a wide concentration range 3.98 x 10 ( -6 ) to 1.0 x 10 ( -1 ) M with a slope of 29.0 + / -0.1 mV/decade of concentration and a detection limit of 2.82 x 10 ( -6 ) M. It showed a response time of less than 10s and could be used for at least 3 months without any divergence in potential .
	manualset3
148640	2	409829	5	NULL	NULL	0	NULL	Nernstian response	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrode exhibited a Nernstian response for strontium ion over a wide concentration range 3.98 x 10 ( -6 ) to 1.0 x 10 ( -1 ) M with a slope of 29.0 + / -0.1 mV/decade of concentration and a detection limit of 2.82 x 10 ( -6 ) M. It showed a response time of less than 10s and could be used for at least 3 months without any divergence in potential .
	manualset3
148641	3	409829	5	NULL	NULL	0	NULL	strontium ion	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrode exhibited a Nernstian response for strontium ion over a wide concentration range 3.98 x 10 ( -6 ) to 1.0 x 10 ( -1 ) M with a slope of 29.0 + / -0.1 mV/decade of concentration and a detection limit of 2.82 x 10 ( -6 ) M. It showed a response time of less than 10s and could be used for at least 3 months without any divergence in potential .
	manualset3
148642	4	409829	5	NULL	NULL	0	NULL	concentration range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrode exhibited a Nernstian response for strontium ion over a wide concentration range 3.98 x 10 ( -6 ) to 1.0 x 10 ( -1 ) M with a slope of 29.0 + / -0.1 mV/decade of concentration and a detection limit of 2.82 x 10 ( -6 ) M. It showed a response time of less than 10s and could be used for at least 3 months without any divergence in potential .
	manualset3
148643	5	409829	5	NULL	NULL	0	NULL	3.98 x 10 ( -6 ) to 1.0 x 10 ( -1 ) M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrode exhibited a Nernstian response for strontium ion over a wide concentration range 3.98 x 10 ( -6 ) to 1.0 x 10 ( -1 ) M with a slope of 29.0 + / -0.1 mV/decade of concentration and a detection limit of 2.82 x 10 ( -6 ) M. It showed a response time of less than 10s and could be used for at least 3 months without any divergence in potential .
	manualset3
148644	6	409829	5	NULL	NULL	0	NULL	slope 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrode exhibited a Nernstian response for strontium ion over a wide concentration range 3.98 x 10 ( -6 ) to 1.0 x 10 ( -1 ) M with a slope of 29.0 + / -0.1 mV/decade of concentration and a detection limit of 2.82 x 10 ( -6 ) M. It showed a response time of less than 10s and could be used for at least 3 months without any divergence in potential .
	manualset3
148645	7	409829	5	NULL	NULL	0	NULL	29.0 + / -0.1 mV/decade	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrode exhibited a Nernstian response for strontium ion over a wide concentration range 3.98 x 10 ( -6 ) to 1.0 x 10 ( -1 ) M with a slope of 29.0 + / -0.1 mV/decade of concentration and a detection limit of 2.82 x 10 ( -6 ) M. It showed a response time of less than 10s and could be used for at least 3 months without any divergence in potential .
	manualset3
148646	8	409829	5	NULL	NULL	0	NULL	concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrode exhibited a Nernstian response for strontium ion over a wide concentration range 3.98 x 10 ( -6 ) to 1.0 x 10 ( -1 ) M with a slope of 29.0 + / -0.1 mV/decade of concentration and a detection limit of 2.82 x 10 ( -6 ) M. It showed a response time of less than 10s and could be used for at least 3 months without any divergence in potential .
	manualset3
148647	9	409829	5	NULL	NULL	0	NULL	detection limit 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrode exhibited a Nernstian response for strontium ion over a wide concentration range 3.98 x 10 ( -6 ) to 1.0 x 10 ( -1 ) M with a slope of 29.0 + / -0.1 mV/decade of concentration and a detection limit of 2.82 x 10 ( -6 ) M. It showed a response time of less than 10s and could be used for at least 3 months without any divergence in potential .
	manualset3
148648	10	409829	5	NULL	NULL	0	NULL	2.82 x 10 ( -6 ) M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrode exhibited a Nernstian response for strontium ion over a wide concentration range 3.98 x 10 ( -6 ) to 1.0 x 10 ( -1 ) M with a slope of 29.0 + / -0.1 mV/decade of concentration and a detection limit of 2.82 x 10 ( -6 ) M. It showed a response time of less than 10s and could be used for at least 3 months without any divergence in potential .
	manualset3
148649	11	409829	5	NULL	NULL	0	NULL	response time 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrode exhibited a Nernstian response for strontium ion over a wide concentration range 3.98 x 10 ( -6 ) to 1.0 x 10 ( -1 ) M with a slope of 29.0 + / -0.1 mV/decade of concentration and a detection limit of 2.82 x 10 ( -6 ) M. It showed a response time of less than 10s and could be used for at least 3 months without any divergence in potential .
	manualset3
148650	12	409829	5	NULL	NULL	0	NULL	10s	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrode exhibited a Nernstian response for strontium ion over a wide concentration range 3.98 x 10 ( -6 ) to 1.0 x 10 ( -1 ) M with a slope of 29.0 + / -0.1 mV/decade of concentration and a detection limit of 2.82 x 10 ( -6 ) M. It showed a response time of less than 10s and could be used for at least 3 months without any divergence in potential .
	manualset3
148651	13	409829	5	NULL	NULL	0	NULL	3 months 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrode exhibited a Nernstian response for strontium ion over a wide concentration range 3.98 x 10 ( -6 ) to 1.0 x 10 ( -1 ) M with a slope of 29.0 + / -0.1 mV/decade of concentration and a detection limit of 2.82 x 10 ( -6 ) M. It showed a response time of less than 10s and could be used for at least 3 months without any divergence in potential .
	manualset3
148652	14	409829	5	NULL	NULL	0	NULL	divergence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrode exhibited a Nernstian response for strontium ion over a wide concentration range 3.98 x 10 ( -6 ) to 1.0 x 10 ( -1 ) M with a slope of 29.0 + / -0.1 mV/decade of concentration and a detection limit of 2.82 x 10 ( -6 ) M. It showed a response time of less than 10s and could be used for at least 3 months without any divergence in potential .
	manualset3
148653	15	409829	5	NULL	NULL	0	NULL	potential 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrode exhibited a Nernstian response for strontium ion over a wide concentration range 3.98 x 10 ( -6 ) to 1.0 x 10 ( -1 ) M with a slope of 29.0 + / -0.1 mV/decade of concentration and a detection limit of 2.82 x 10 ( -6 ) M. It showed a response time of less than 10s and could be used for at least 3 months without any divergence in potential .
	manualset3
148654	1	409830	5	NULL	NULL	NULL	NULL	electrodeposition 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The electrodeposition of Pt nanoparticles could be carried out on a GC electrode in DEMEBF ( 4 ) containing ( PtCl ( 6 ) ) ( 2 - ) by holding the potential at -3.5 or -2.0 V. At -3.5 V , the four-electron reduction of ( PtCl ( 6 ) ) ( 2 - ) to Pt can take place , while at -2.0 V the two-electron reduction of ( PtCl ( 6 ) ) ( 2 - ) to ( PtCl ( 4 ) ) ( 2 - ) occurs .
	manualset3
148655	2	409830	5	NULL	NULL	0	NULL	Pt nanoparticles 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrodeposition of Pt nanoparticles could be carried out on a GC electrode in DEMEBF ( 4 ) containing ( PtCl ( 6 ) ) ( 2 - ) by holding the potential at -3.5 or -2.0 V. At -3.5 V , the four-electron reduction of ( PtCl ( 6 ) ) ( 2 - ) to Pt can take place , while at -2.0 V the two-electron reduction of ( PtCl ( 6 ) ) ( 2 - ) to ( PtCl ( 4 ) ) ( 2 - ) occurs .
	manualset3
148656	3	409830	5	NULL	NULL	0	NULL	GC electrode	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrodeposition of Pt nanoparticles could be carried out on a GC electrode in DEMEBF ( 4 ) containing ( PtCl ( 6 ) ) ( 2 - ) by holding the potential at -3.5 or -2.0 V. At -3.5 V , the four-electron reduction of ( PtCl ( 6 ) ) ( 2 - ) to Pt can take place , while at -2.0 V the two-electron reduction of ( PtCl ( 6 ) ) ( 2 - ) to ( PtCl ( 4 ) ) ( 2 - ) occurs .
	manualset3
148657	4	409830	5	NULL	NULL	0	NULL	DEMEBF ( 4 ) 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrodeposition of Pt nanoparticles could be carried out on a GC electrode in DEMEBF ( 4 ) containing ( PtCl ( 6 ) ) ( 2 - ) by holding the potential at -3.5 or -2.0 V. At -3.5 V , the four-electron reduction of ( PtCl ( 6 ) ) ( 2 - ) to Pt can take place , while at -2.0 V the two-electron reduction of ( PtCl ( 6 ) ) ( 2 - ) to ( PtCl ( 4 ) ) ( 2 - ) occurs .
	manualset3
148658	5	409830	5	NULL	NULL	0	NULL	( PtCl ( 6 ) ) ( 2 - ) 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrodeposition of Pt nanoparticles could be carried out on a GC electrode in DEMEBF ( 4 ) containing ( PtCl ( 6 ) ) ( 2 - ) by holding the potential at -3.5 or -2.0 V. At -3.5 V , the four-electron reduction of ( PtCl ( 6 ) ) ( 2 - ) to Pt can take place , while at -2.0 V the two-electron reduction of ( PtCl ( 6 ) ) ( 2 - ) to ( PtCl ( 4 ) ) ( 2 - ) occurs .
	manualset3
148659	6	409830	5	NULL	NULL	0	NULL	potential 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrodeposition of Pt nanoparticles could be carried out on a GC electrode in DEMEBF ( 4 ) containing ( PtCl ( 6 ) ) ( 2 - ) by holding the potential at -3.5 or -2.0 V. At -3.5 V , the four-electron reduction of ( PtCl ( 6 ) ) ( 2 - ) to Pt can take place , while at -2.0 V the two-electron reduction of ( PtCl ( 6 ) ) ( 2 - ) to ( PtCl ( 4 ) ) ( 2 - ) occurs .
	manualset3
148660	7	409830	5	NULL	NULL	0	NULL	-3.5 or -2.0 V	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrodeposition of Pt nanoparticles could be carried out on a GC electrode in DEMEBF ( 4 ) containing ( PtCl ( 6 ) ) ( 2 - ) by holding the potential at -3.5 or -2.0 V. At -3.5 V , the four-electron reduction of ( PtCl ( 6 ) ) ( 2 - ) to Pt can take place , while at -2.0 V the two-electron reduction of ( PtCl ( 6 ) ) ( 2 - ) to ( PtCl ( 4 ) ) ( 2 - ) occurs .
	manualset3
148661	8	409830	5	NULL	NULL	0	NULL	 -3.5 V	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrodeposition of Pt nanoparticles could be carried out on a GC electrode in DEMEBF ( 4 ) containing ( PtCl ( 6 ) ) ( 2 - ) by holding the potential at -3.5 or -2.0 V. At -3.5 V , the four-electron reduction of ( PtCl ( 6 ) ) ( 2 - ) to Pt can take place , while at -2.0 V the two-electron reduction of ( PtCl ( 6 ) ) ( 2 - ) to ( PtCl ( 4 ) ) ( 2 - ) occurs .
	manualset3
148662	9	409830	5	NULL	NULL	0	NULL	four-electron reduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrodeposition of Pt nanoparticles could be carried out on a GC electrode in DEMEBF ( 4 ) containing ( PtCl ( 6 ) ) ( 2 - ) by holding the potential at -3.5 or -2.0 V. At -3.5 V , the four-electron reduction of ( PtCl ( 6 ) ) ( 2 - ) to Pt can take place , while at -2.0 V the two-electron reduction of ( PtCl ( 6 ) ) ( 2 - ) to ( PtCl ( 4 ) ) ( 2 - ) occurs .
	manualset3
148663	10	409830	5	NULL	NULL	0	NULL	( PtCl ( 6 ) ) ( 2 - )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrodeposition of Pt nanoparticles could be carried out on a GC electrode in DEMEBF ( 4 ) containing ( PtCl ( 6 ) ) ( 2 - ) by holding the potential at -3.5 or -2.0 V. At -3.5 V , the four-electron reduction of ( PtCl ( 6 ) ) ( 2 - ) to Pt can take place , while at -2.0 V the two-electron reduction of ( PtCl ( 6 ) ) ( 2 - ) to ( PtCl ( 4 ) ) ( 2 - ) occurs .
	manualset3
148664	11	409830	5	NULL	NULL	0	NULL	Pt	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrodeposition of Pt nanoparticles could be carried out on a GC electrode in DEMEBF ( 4 ) containing ( PtCl ( 6 ) ) ( 2 - ) by holding the potential at -3.5 or -2.0 V. At -3.5 V , the four-electron reduction of ( PtCl ( 6 ) ) ( 2 - ) to Pt can take place , while at -2.0 V the two-electron reduction of ( PtCl ( 6 ) ) ( 2 - ) to ( PtCl ( 4 ) ) ( 2 - ) occurs .
	manualset3
148665	12	409830	5	NULL	NULL	0	NULL	-2.0 V	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrodeposition of Pt nanoparticles could be carried out on a GC electrode in DEMEBF ( 4 ) containing ( PtCl ( 6 ) ) ( 2 - ) by holding the potential at -3.5 or -2.0 V. At -3.5 V , the four-electron reduction of ( PtCl ( 6 ) ) ( 2 - ) to Pt can take place , while at -2.0 V the two-electron reduction of ( PtCl ( 6 ) ) ( 2 - ) to ( PtCl ( 4 ) ) ( 2 - ) occurs .
	manualset3
148666	13	409830	5	NULL	NULL	0	NULL	two-electron reduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrodeposition of Pt nanoparticles could be carried out on a GC electrode in DEMEBF ( 4 ) containing ( PtCl ( 6 ) ) ( 2 - ) by holding the potential at -3.5 or -2.0 V. At -3.5 V , the four-electron reduction of ( PtCl ( 6 ) ) ( 2 - ) to Pt can take place , while at -2.0 V the two-electron reduction of ( PtCl ( 6 ) ) ( 2 - ) to ( PtCl ( 4 ) ) ( 2 - ) occurs .
	manualset3
148667	14	409830	5	NULL	NULL	NULL	NULL	( PtCl ( 6 ) ) ( 2 - ) to ( PtCl ( 4 ) ) ( 2 - ) 	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The electrodeposition of Pt nanoparticles could be carried out on a GC electrode in DEMEBF ( 4 ) containing ( PtCl ( 6 ) ) ( 2 - ) by holding the potential at -3.5 or -2.0 V. At -3.5 V , the four-electron reduction of ( PtCl ( 6 ) ) ( 2 - ) to Pt can take place , while at -2.0 V the two-electron reduction of ( PtCl ( 6 ) ) ( 2 - ) to ( PtCl ( 4 ) ) ( 2 - ) occurs .
	manualset3
148915	1	409831	7	NULL	NULL	0	NULL	electron coupling 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The electron coupling between the protonated amine groups of phospholipids and PAHs in chloroform was verified by the electronic deshielding-induced downfield chemical shifts of phenanthrene at low pH in the 1H NMR spectrum .
	manualset3
148916	2	409831	7	NULL	NULL	0	NULL	protonated amine groups of phospholipids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The electron coupling between the protonated amine groups of phospholipids and PAHs in chloroform was verified by the electronic deshielding-induced downfield chemical shifts of phenanthrene at low pH in the 1H NMR spectrum .
	manualset3
148917	3	409831	7	NULL	NULL	0	NULL	PAHs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The electron coupling between the protonated amine groups of phospholipids and PAHs in chloroform was verified by the electronic deshielding-induced downfield chemical shifts of phenanthrene at low pH in the 1H NMR spectrum .
	manualset3
148918	4	409831	7	NULL	NULL	NULL	NULL	electronic deshielding-induced downfield chemical shifts	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The electron coupling between the protonated amine groups of phospholipids and PAHs in chloroform was verified by the electronic deshielding-induced downfield chemical shifts of phenanthrene at low pH in the 1H NMR spectrum .
	manualset3
148919	5	409831	7	NULL	NULL	0	NULL	phenanthrene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The electron coupling between the protonated amine groups of phospholipids and PAHs in chloroform was verified by the electronic deshielding-induced downfield chemical shifts of phenanthrene at low pH in the 1H NMR spectrum .
	manualset3
148927	6	409831	7	NULL	NULL	NULL	NULL	low pH	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The electron coupling between the protonated amine groups of phospholipids and PAHs in chloroform was verified by the electronic deshielding-induced downfield chemical shifts of phenanthrene at low pH in the 1H NMR spectrum .
	manualset3
148928	7	409831	7	NULL	NULL	NULL	NULL	1H NMR spectrum	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The electron coupling between the protonated amine groups of phospholipids and PAHs in chloroform was verified by the electronic deshielding-induced downfield chemical shifts of phenanthrene at low pH in the 1H NMR spectrum .
	manualset3
148936	2	409832	7	NULL	NULL	NULL	NULL	spinal cord evoked potentials ( SCEPs )	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The electrophysiological measurement of spinal cord evoked potentials ( SCEPs ) has been established as a tool for diagnosing the spinal level responsible for cervical myelopathy .
	manualset3
148939	4	409832	7	NULL	NULL	NULL	NULL	spinal level	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The electrophysiological measurement of spinal cord evoked potentials ( SCEPs ) has been established as a tool for diagnosing the spinal level responsible for cervical myelopathy .
	manualset3
148940	5	409832	7	NULL	NULL	NULL	NULL	cervical myelopathy	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The electrophysiological measurement of spinal cord evoked potentials ( SCEPs ) has been established as a tool for diagnosing the spinal level responsible for cervical myelopathy .
	manualset3
149210	1	409832	7	NULL	NULL	NULL	NULL	electrophysiological measurement	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The electrophysiological measurement of spinal cord evoked potentials ( SCEPs ) has been established as a tool for diagnosing the spinal level responsible for cervical myelopathy .
	manualset3
149211	3	409832	7	NULL	NULL	NULL	NULL	 tool	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The electrophysiological measurement of spinal cord evoked potentials ( SCEPs ) has been established as a tool for diagnosing the spinal level responsible for cervical myelopathy .
	manualset3
148941	2	409833	7	NULL	NULL	NULL	NULL	UDP-N-acetylhexosamine	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The elevated cytosolic level of UDP-N-acetylhexosamine ( and of compounds like CMP ) is suggested to impair the transport of CMP-acetylneuraminate to the Golgi , resulting in reduced sialylation .
	manualset3
148942	4	409833	7	NULL	NULL	NULL	NULL	transport	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The elevated cytosolic level of UDP-N-acetylhexosamine ( and of compounds like CMP ) is suggested to impair the transport of CMP-acetylneuraminate to the Golgi , resulting in reduced sialylation .
	manualset3
148943	5	409833	7	NULL	NULL	NULL	NULL	CMP-acetylneuraminate	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The elevated cytosolic level of UDP-N-acetylhexosamine ( and of compounds like CMP ) is suggested to impair the transport of CMP-acetylneuraminate to the Golgi , resulting in reduced sialylation .
	manualset3
148944	6	409833	7	NULL	NULL	NULL	NULL	Golgi	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The elevated cytosolic level of UDP-N-acetylhexosamine ( and of compounds like CMP ) is suggested to impair the transport of CMP-acetylneuraminate to the Golgi , resulting in reduced sialylation .
	manualset3
148945	7	409833	7	NULL	NULL	NULL	NULL	reduced sialylation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The elevated cytosolic level of UDP-N-acetylhexosamine ( and of compounds like CMP ) is suggested to impair the transport of CMP-acetylneuraminate to the Golgi , resulting in reduced sialylation .
	manualset3
149212	1	409833	7	NULL	NULL	NULL	NULL	elevated cytosolic level	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The elevated cytosolic level of UDP-N-acetylhexosamine ( and of compounds like CMP ) is suggested to impair the transport of CMP-acetylneuraminate to the Golgi , resulting in reduced sialylation .
	manualset3
149213	3	409833	7	NULL	NULL	0	NULL	 CMP 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The elevated cytosolic level of UDP-N-acetylhexosamine ( and of compounds like CMP ) is suggested to impair the transport of CMP-acetylneuraminate to the Golgi , resulting in reduced sialylation .
	manualset3
148970	1	409834	7	NULL	NULL	NULL	NULL	elevations in pressure 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The elevations in pressure were associated with high resting central blood volumes which increased significantly with exertion .
	manualset3
148975	2	409834	7	NULL	NULL	NULL	NULL	high resting central blood volumes	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The elevations in pressure were associated with high resting central blood volumes which increased significantly with exertion .
	manualset3
148976	3	409834	7	NULL	NULL	0	NULL	exertion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The elevations in pressure were associated with high resting central blood volumes which increased significantly with exertion .
	manualset3
148977	1	409835	7	NULL	NULL	NULL	NULL	ellipsometry measurements	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ellipsometry measurements on these specimens were carried out at a number of angles of incidence in the 30-80 degrees range and at a number of discrete wavelengths in the 300-650-nm spectral range .
	manualset3
149011	2	409835	7	NULL	NULL	0	NULL	specimens	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ellipsometry measurements on these specimens were carried out at a number of angles of incidence in the 30-80 degrees range and at a number of discrete wavelengths in the 300-650-nm spectral range .
	manualset3
149016	4	409835	7	NULL	NULL	NULL	NULL	30-80 degrees range	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ellipsometry measurements on these specimens were carried out at a number of angles of incidence in the 30-80 degrees range and at a number of discrete wavelengths in the 300-650-nm spectral range .
	manualset3
149022	5	409835	7	NULL	NULL	NULL	NULL	discrete wavelengths	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ellipsometry measurements on these specimens were carried out at a number of angles of incidence in the 30-80 degrees range and at a number of discrete wavelengths in the 300-650-nm spectral range .
	manualset3
149214	6	409835	7	NULL	NULL	NULL	NULL	300-650-nm spectral range	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ellipsometry measurements on these specimens were carried out at a number of angles of incidence in the 30-80 degrees range and at a number of discrete wavelengths in the 300-650-nm spectral range .
	manualset3
149804	3	409835	7	NULL	NULL	0	NULL	angles of incidence	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The ellipsometry measurements on these specimens were carried out at a number of angles of incidence in the 30-80 degrees range and at a number of discrete wavelengths in the 300-650-nm spectral range .
	manualset3
149023	1	409836	7	NULL	NULL	0	NULL	elusive marrow toxin	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The elusive marrow toxin -- neutropenia of West Indians .
	manualset3
149024	2	409836	7	NULL	NULL	0	NULL	neutropenia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The elusive marrow toxin -- neutropenia of West Indians .
	manualset3
149025	3	409836	7	NULL	NULL	0	NULL	West Indians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The elusive marrow toxin -- neutropenia of West Indians .
	manualset3
149026	1	409837	7	NULL	NULL	0	NULL	complete polysaccharide component	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A structure is proposed for the complete polysaccharide component of the smooth-form lipopolysaccharide comprising the O antigen chain , an intervening region , and the inner core oligosaccharide on the basis of 1H and 13C NMR experiments , fast atom bombardment/mass spectrometry , and methylation linkage analysis of permethylated oligo - and polysaccharide derivatives .
	manualset3
149027	2	409837	7	NULL	NULL	0	NULL	smooth-form lipopolysaccharide 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A structure is proposed for the complete polysaccharide component of the smooth-form lipopolysaccharide comprising the O antigen chain , an intervening region , and the inner core oligosaccharide on the basis of 1H and 13C NMR experiments , fast atom bombardment/mass spectrometry , and methylation linkage analysis of permethylated oligo - and polysaccharide derivatives .
	manualset3
149031	3	409837	7	NULL	NULL	NULL	NULL	O antigen chain	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A structure is proposed for the complete polysaccharide component of the smooth-form lipopolysaccharide comprising the O antigen chain , an intervening region , and the inner core oligosaccharide on the basis of 1H and 13C NMR experiments , fast atom bombardment/mass spectrometry , and methylation linkage analysis of permethylated oligo - and polysaccharide derivatives .
	manualset3
149032	4	409837	7	NULL	NULL	0	NULL	inner core oligosaccharide	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A structure is proposed for the complete polysaccharide component of the smooth-form lipopolysaccharide comprising the O antigen chain , an intervening region , and the inner core oligosaccharide on the basis of 1H and 13C NMR experiments , fast atom bombardment/mass spectrometry , and methylation linkage analysis of permethylated oligo - and polysaccharide derivatives .
	manualset3
149033	5	409837	7	NULL	NULL	0	NULL	1H and 13C NMR experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A structure is proposed for the complete polysaccharide component of the smooth-form lipopolysaccharide comprising the O antigen chain , an intervening region , and the inner core oligosaccharide on the basis of 1H and 13C NMR experiments , fast atom bombardment/mass spectrometry , and methylation linkage analysis of permethylated oligo - and polysaccharide derivatives .
	manualset3
149034	6	409837	7	NULL	NULL	0	NULL	fast atom bombardment/mass spectrometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A structure is proposed for the complete polysaccharide component of the smooth-form lipopolysaccharide comprising the O antigen chain , an intervening region , and the inner core oligosaccharide on the basis of 1H and 13C NMR experiments , fast atom bombardment/mass spectrometry , and methylation linkage analysis of permethylated oligo - and polysaccharide derivatives .
	manualset3
149035	7	409837	7	NULL	NULL	0	NULL	methylation linkage analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A structure is proposed for the complete polysaccharide component of the smooth-form lipopolysaccharide comprising the O antigen chain , an intervening region , and the inner core oligosaccharide on the basis of 1H and 13C NMR experiments , fast atom bombardment/mass spectrometry , and methylation linkage analysis of permethylated oligo - and polysaccharide derivatives .
	manualset3
149036	8	409837	7	NULL	NULL	0	NULL	permethylated oligo - and polysaccharide derivatives	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A structure is proposed for the complete polysaccharide component of the smooth-form lipopolysaccharide comprising the O antigen chain , an intervening region , and the inner core oligosaccharide on the basis of 1H and 13C NMR experiments , fast atom bombardment/mass spectrometry , and methylation linkage analysis of permethylated oligo - and polysaccharide derivatives .
	manualset3
149037	1	409838	7	NULL	NULL	NULL	NULL	elute	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The elute was shown by negative-stain electron microscopy to contain purified acidosomes ( saccular membranes studded with V-H ( + ) - ATPase ) .
	manualset3
149038	2	409838	7	NULL	NULL	0	NULL	negative-stain electron microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The elute was shown by negative-stain electron microscopy to contain purified acidosomes ( saccular membranes studded with V-H ( + ) - ATPase ) .
	manualset3
149039	3	409838	7	NULL	NULL	0	NULL	purified acidosomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The elute was shown by negative-stain electron microscopy to contain purified acidosomes ( saccular membranes studded with V-H ( + ) - ATPase ) .
	manualset3
149040	4	409838	7	NULL	NULL	0	NULL	saccular membranes 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The elute was shown by negative-stain electron microscopy to contain purified acidosomes ( saccular membranes studded with V-H ( + ) - ATPase ) .
	manualset3
149041	5	409838	7	NULL	NULL	0	NULL	V-H ( + ) - ATPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The elute was shown by negative-stain electron microscopy to contain purified acidosomes ( saccular membranes studded with V-H ( + ) - ATPase ) .
	manualset3
149047	1	409839	7	NULL	NULL	0	NULL	embryos of teleost fish 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The embryos of teleost fish are exquisitely sensitive to the toxic effects of exposure to 2 , 3 , 7 , 8-tetrachlorodibenzo-p-dioxin ( TCDD ) .
	manualset3
149048	2	409839	7	NULL	NULL	NULL	NULL	toxic effects	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The embryos of teleost fish are exquisitely sensitive to the toxic effects of exposure to 2 , 3 , 7 , 8-tetrachlorodibenzo-p-dioxin ( TCDD ) .
	manualset3
149050	4	409839	7	NULL	NULL	NULL	NULL	2 , 3 , 7 , 8-tetrachlorodibenzo-p-dioxin	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The embryos of teleost fish are exquisitely sensitive to the toxic effects of exposure to 2 , 3 , 7 , 8-tetrachlorodibenzo-p-dioxin ( TCDD ) .
	manualset3
149215	3	409839	7	NULL	NULL	0	NULL	exposure	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The embryos of teleost fish are exquisitely sensitive to the toxic effects of exposure to 2 , 3 , 7 , 8-tetrachlorodibenzo-p-dioxin ( TCDD ) .
	manualset3
149051	1	409840	7	NULL	NULL	0	NULL	embryos	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The embryos were dechorionated at 4 h post fertilization ( hpf ) and irradiated at 5 hpf by microbeam protons .
	manualset3
149057	3	409840	7	NULL	NULL	NULL	NULL	4 h post fertilization ( hpf )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The embryos were dechorionated at 4 h post fertilization ( hpf ) and irradiated at 5 hpf by microbeam protons .
	manualset3
149058	4	409840	7	NULL	NULL	0	NULL	5 hpf	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The embryos were dechorionated at 4 h post fertilization ( hpf ) and irradiated at 5 hpf by microbeam protons .
	manualset3
149059	5	409840	7	NULL	NULL	0	NULL	microbeam protons	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The embryos were dechorionated at 4 h post fertilization ( hpf ) and irradiated at 5 hpf by microbeam protons .
	manualset3
149216	2	409841	7	NULL	NULL	NULL	NULL	adamantane-resistant H3N2 viruses	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The emergence and global spread of adamantane-resistant H3N2 viruses in 2003-2004 and oseltamivir-resistant seasonal H1N1 viruses in 2007-2009 demonstrated the ability of drug-resistant variants to rapidly become predominant worldwide .
	manualset3
149217	4	409841	7	NULL	NULL	NULL	NULL	oseltamivir-resistant seasonal H1N1 viruses	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The emergence and global spread of adamantane-resistant H3N2 viruses in 2003-2004 and oseltamivir-resistant seasonal H1N1 viruses in 2007-2009 demonstrated the ability of drug-resistant variants to rapidly become predominant worldwide .
	manualset3
149218	6	409841	7	NULL	NULL	NULL	NULL	drug-resistant variants	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The emergence and global spread of adamantane-resistant H3N2 viruses in 2003-2004 and oseltamivir-resistant seasonal H1N1 viruses in 2007-2009 demonstrated the ability of drug-resistant variants to rapidly become predominant worldwide .
	manualset3
149219	1	409841	7	NULL	NULL	NULL	NULL	emergence and global spread 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The emergence and global spread of adamantane-resistant H3N2 viruses in 2003-2004 and oseltamivir-resistant seasonal H1N1 viruses in 2007-2009 demonstrated the ability of drug-resistant variants to rapidly become predominant worldwide .
	manualset3
149514	3	409841	7	NULL	NULL	0	NULL	2003-2004	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The emergence and global spread of adamantane-resistant H3N2 viruses in 2003-2004 and oseltamivir-resistant seasonal H1N1 viruses in 2007-2009 demonstrated the ability of drug-resistant variants to rapidly become predominant worldwide .
	manualset3
149517	5	409841	7	NULL	NULL	NULL	NULL	 2007-2009	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The emergence and global spread of adamantane-resistant H3N2 viruses in 2003-2004 and oseltamivir-resistant seasonal H1N1 viruses in 2007-2009 demonstrated the ability of drug-resistant variants to rapidly become predominant worldwide .
	manualset3
149221	1	409842	7	NULL	NULL	0	NULL	emergence of a migration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The emergence of a migration was predicted to be dependent on the ability of the wildebeest to track changes in resource abundance at relatively large scales ( ) 80-100 km ) .
	manualset3
149222	3	409842	7	NULL	NULL	NULL	NULL	 wildebeest	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The emergence of a migration was predicted to be dependent on the ability of the wildebeest to track changes in resource abundance at relatively large scales ( ) 80-100 km ) .
	manualset3
149224	4	409842	7	NULL	NULL	NULL	NULL	 changes	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The emergence of a migration was predicted to be dependent on the ability of the wildebeest to track changes in resource abundance at relatively large scales ( ) 80-100 km ) .
	manualset3
149225	5	409842	7	NULL	NULL	0	NULL	resource abundance 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The emergence of a migration was predicted to be dependent on the ability of the wildebeest to track changes in resource abundance at relatively large scales ( ) 80-100 km ) .
	manualset3
149226	6	409842	7	NULL	NULL	NULL	NULL	large scales	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The emergence of a migration was predicted to be dependent on the ability of the wildebeest to track changes in resource abundance at relatively large scales ( ) 80-100 km ) .
	manualset3
149227	7	409842	7	NULL	NULL	0	NULL	80-100 km	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The emergence of a migration was predicted to be dependent on the ability of the wildebeest to track changes in resource abundance at relatively large scales ( ) 80-100 km ) .
	manualset3
149228	1	409843	7	NULL	NULL	NULL	NULL	emergence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The emergence of multidrug-resistant strains of Salmonella , leading to increased morbidity and mortality , has further complicated its management .
	manualset3
149229	2	409843	7	NULL	NULL	0	NULL	multidrug-resistant strains of Salmonella	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The emergence of multidrug-resistant strains of Salmonella , leading to increased morbidity and mortality , has further complicated its management .
	manualset3
149230	3	409843	7	NULL	NULL	0	NULL	 increased morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The emergence of multidrug-resistant strains of Salmonella , leading to increased morbidity and mortality , has further complicated its management .
	manualset3
149231	4	409843	7	NULL	NULL	NULL	NULL	increased mortality	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The emergence of multidrug-resistant strains of Salmonella , leading to increased morbidity and mortality , has further complicated its management .
	manualset3
157156	5	409843	7	NULL	NULL	0	NULL	management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The emergence of multidrug-resistant strains of Salmonella , leading to increased morbidity and mortality , has further complicated its management .
	manualset3
149232	1	409844	7	NULL	NULL	0	NULL	emergence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The emergence of spike-firing pattern and the underlying ion channels were studied in morphologically-identified principal cells using whole-cell patch-clamp recordings from brain slices of late-term embryos ( embryonic day 16 ) and hatchling chickens ( hatching day 1 and hatching day 5 ) .
	manualset3
149233	2	409844	7	NULL	NULL	NULL	NULL	spike-firing pattern 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The emergence of spike-firing pattern and the underlying ion channels were studied in morphologically-identified principal cells using whole-cell patch-clamp recordings from brain slices of late-term embryos ( embryonic day 16 ) and hatchling chickens ( hatching day 1 and hatching day 5 ) .
	manualset3
149234	3	409844	7	NULL	NULL	NULL	NULL	 underlying ion channels	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The emergence of spike-firing pattern and the underlying ion channels were studied in morphologically-identified principal cells using whole-cell patch-clamp recordings from brain slices of late-term embryos ( embryonic day 16 ) and hatchling chickens ( hatching day 1 and hatching day 5 ) .
	manualset3
149235	4	409844	7	NULL	NULL	0	NULL	morphologically-identified principal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The emergence of spike-firing pattern and the underlying ion channels were studied in morphologically-identified principal cells using whole-cell patch-clamp recordings from brain slices of late-term embryos ( embryonic day 16 ) and hatchling chickens ( hatching day 1 and hatching day 5 ) .
	manualset3
149236	5	409844	7	NULL	NULL	0	NULL	whole-cell patch-clamp recordings	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The emergence of spike-firing pattern and the underlying ion channels were studied in morphologically-identified principal cells using whole-cell patch-clamp recordings from brain slices of late-term embryos ( embryonic day 16 ) and hatchling chickens ( hatching day 1 and hatching day 5 ) .
	manualset3
149237	6	409844	7	NULL	NULL	0	NULL	 brain slices	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The emergence of spike-firing pattern and the underlying ion channels were studied in morphologically-identified principal cells using whole-cell patch-clamp recordings from brain slices of late-term embryos ( embryonic day 16 ) and hatchling chickens ( hatching day 1 and hatching day 5 ) .
	manualset3
149238	7	409844	7	NULL	NULL	0	NULL	late-term embryos 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The emergence of spike-firing pattern and the underlying ion channels were studied in morphologically-identified principal cells using whole-cell patch-clamp recordings from brain slices of late-term embryos ( embryonic day 16 ) and hatchling chickens ( hatching day 1 and hatching day 5 ) .
	manualset3
149239	8	409844	7	NULL	NULL	NULL	NULL	embryonic day 16 	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The emergence of spike-firing pattern and the underlying ion channels were studied in morphologically-identified principal cells using whole-cell patch-clamp recordings from brain slices of late-term embryos ( embryonic day 16 ) and hatchling chickens ( hatching day 1 and hatching day 5 ) .
	manualset3
149240	9	409844	7	NULL	NULL	0	NULL	hatchling chickens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The emergence of spike-firing pattern and the underlying ion channels were studied in morphologically-identified principal cells using whole-cell patch-clamp recordings from brain slices of late-term embryos ( embryonic day 16 ) and hatchling chickens ( hatching day 1 and hatching day 5 ) .
	manualset3
149241	10	409844	7	NULL	NULL	NULL	NULL	hatching day 1 	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The emergence of spike-firing pattern and the underlying ion channels were studied in morphologically-identified principal cells using whole-cell patch-clamp recordings from brain slices of late-term embryos ( embryonic day 16 ) and hatchling chickens ( hatching day 1 and hatching day 5 ) .
	manualset3
149242	11	409844	7	NULL	NULL	NULL	NULL	hatching day 5 	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The emergence of spike-firing pattern and the underlying ion channels were studied in morphologically-identified principal cells using whole-cell patch-clamp recordings from brain slices of late-term embryos ( embryonic day 16 ) and hatchling chickens ( hatching day 1 and hatching day 5 ) .
	manualset3
149243	1	409845	7	NULL	NULL	0	NULL	emerging role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The emerging role of echocardiography in the emergency department .
	manualset3
149244	2	409845	7	NULL	NULL	NULL	NULL	echocardiography	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The emerging role of echocardiography in the emergency department .
	manualset3
149245	3	409845	7	NULL	NULL	0	NULL	emergency department	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The emerging role of echocardiography in the emergency department .
	manualset3
149246	1	409846	7	NULL	NULL	0	NULL	emission	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The emission at 450 + / - 10 nm , excited at 360 nm , provides a measure of NADH ( and NADPH ) per cell .
	manualset3
149247	2	409846	7	NULL	NULL	0	NULL	450 + / - 10 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The emission at 450 + / - 10 nm , excited at 360 nm , provides a measure of NADH ( and NADPH ) per cell .
	manualset3
149248	3	409846	7	NULL	NULL	NULL	NULL	 360 nm	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The emission at 450 + / - 10 nm , excited at 360 nm , provides a measure of NADH ( and NADPH ) per cell .
	manualset3
149249	4	409846	7	NULL	NULL	NULL	NULL	NADH 	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The emission at 450 + / - 10 nm , excited at 360 nm , provides a measure of NADH ( and NADPH ) per cell .
	manualset3
149250	5	409846	7	NULL	NULL	NULL	NULL	NADPH  per cell	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The emission at 450 + / - 10 nm , excited at 360 nm , provides a measure of NADH ( and NADPH ) per cell .
	manualset3
149251	1	409847	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A study by a Minnesota health plan shows that , on average , a victim of domestic violence costs the health care system $ 1 , 434 more per year than a nonvictim .
	manualset3
149252	2	409847	7	NULL	NULL	NULL	NULL	Minnesota health plan 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A study by a Minnesota health plan shows that , on average , a victim of domestic violence costs the health care system $ 1 , 434 more per year than a nonvictim .
	manualset3
149253	3	409847	7	NULL	NULL	0	NULL	victim	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A study by a Minnesota health plan shows that , on average , a victim of domestic violence costs the health care system $ 1 , 434 more per year than a nonvictim .
	manualset3
149254	5	409847	7	NULL	NULL	NULL	NULL	health care system	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A study by a Minnesota health plan shows that , on average , a victim of domestic violence costs the health care system $ 1 , 434 more per year than a nonvictim .
	manualset3
149255	6	409847	7	NULL	NULL	NULL	NULL	 $ 1 , 434	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A study by a Minnesota health plan shows that , on average , a victim of domestic violence costs the health care system $ 1 , 434 more per year than a nonvictim .
	manualset3
149256	8	409847	7	NULL	NULL	NULL	NULL	nonvictim	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A study by a Minnesota health plan shows that , on average , a victim of domestic violence costs the health care system $ 1 , 434 more per year than a nonvictim .
	manualset3
149631	4	409847	7	NULL	NULL	NULL	NULL	domestic violence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A study by a Minnesota health plan shows that , on average , a victim of domestic violence costs the health care system $ 1 , 434 more per year than a nonvictim .
	manualset3
149632	7	409847	7	NULL	NULL	0	NULL	per year	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A study by a Minnesota health plan shows that , on average , a victim of domestic violence costs the health care system $ 1 , 434 more per year than a nonvictim .
	manualset3
149257	1	409848	7	NULL	NULL	0	NULL	emission properties	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The emission properties of sparfloxacin and chloro-sparfloxacin are greatly distinct , the fluorescence of sparfloxacin is so weak that it can not be determined by means of fluorescence spectra , but the fluorescence intensity of the new substance is 110 fold more than that of sparfloxacin itself .
	manualset3
149258	2	409848	7	NULL	NULL	0	NULL	sparfloxacin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The emission properties of sparfloxacin and chloro-sparfloxacin are greatly distinct , the fluorescence of sparfloxacin is so weak that it can not be determined by means of fluorescence spectra , but the fluorescence intensity of the new substance is 110 fold more than that of sparfloxacin itself .
	manualset3
149259	3	409848	7	NULL	NULL	0	NULL	chloro-sparfloxacin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The emission properties of sparfloxacin and chloro-sparfloxacin are greatly distinct , the fluorescence of sparfloxacin is so weak that it can not be determined by means of fluorescence spectra , but the fluorescence intensity of the new substance is 110 fold more than that of sparfloxacin itself .
	manualset3
149260	4	409848	7	NULL	NULL	0	NULL	fluorescence of sparfloxacin	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The emission properties of sparfloxacin and chloro-sparfloxacin are greatly distinct , the fluorescence of sparfloxacin is so weak that it can not be determined by means of fluorescence spectra , but the fluorescence intensity of the new substance is 110 fold more than that of sparfloxacin itself .
	manualset3
149261	5	409848	7	NULL	NULL	0	NULL	fluorescence spectra	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The emission properties of sparfloxacin and chloro-sparfloxacin are greatly distinct , the fluorescence of sparfloxacin is so weak that it can not be determined by means of fluorescence spectra , but the fluorescence intensity of the new substance is 110 fold more than that of sparfloxacin itself .
	manualset3
149262	6	409848	7	NULL	NULL	0	NULL	fluorescence intensity	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The emission properties of sparfloxacin and chloro-sparfloxacin are greatly distinct , the fluorescence of sparfloxacin is so weak that it can not be determined by means of fluorescence spectra , but the fluorescence intensity of the new substance is 110 fold more than that of sparfloxacin itself .
	manualset3
149263	7	409848	7	NULL	NULL	NULL	NULL	new substance	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The emission properties of sparfloxacin and chloro-sparfloxacin are greatly distinct , the fluorescence of sparfloxacin is so weak that it can not be determined by means of fluorescence spectra , but the fluorescence intensity of the new substance is 110 fold more than that of sparfloxacin itself .
	manualset3
149264	8	409848	7	NULL	NULL	NULL	NULL	110 fold	Unit												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The emission properties of sparfloxacin and chloro-sparfloxacin are greatly distinct , the fluorescence of sparfloxacin is so weak that it can not be determined by means of fluorescence spectra , but the fluorescence intensity of the new substance is 110 fold more than that of sparfloxacin itself .
	manualset3
149265	9	409848	7	NULL	NULL	0	NULL	sparfloxacin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The emission properties of sparfloxacin and chloro-sparfloxacin are greatly distinct , the fluorescence of sparfloxacin is so weak that it can not be determined by means of fluorescence spectra , but the fluorescence intensity of the new substance is 110 fold more than that of sparfloxacin itself .
	manualset3
149266	1	409849	7	NULL	NULL	0	NULL	employment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The employment of evolving factor analysis and multivariate curve resolution-alternating least squares for decomposition of the series of quantum dots fluorescence spectra recorded by a specific measuring procedure reveals the number of quantum dot fractions having different diameters .
	manualset3
149267	2	409849	7	NULL	NULL	0	NULL	evolving factor analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The employment of evolving factor analysis and multivariate curve resolution-alternating least squares for decomposition of the series of quantum dots fluorescence spectra recorded by a specific measuring procedure reveals the number of quantum dot fractions having different diameters .
	manualset3
149268	3	409849	7	NULL	NULL	NULL	NULL	multivariate curve resolution-alternating least squares	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The employment of evolving factor analysis and multivariate curve resolution-alternating least squares for decomposition of the series of quantum dots fluorescence spectra recorded by a specific measuring procedure reveals the number of quantum dot fractions having different diameters .
	manualset3
149269	4	409849	7	NULL	NULL	0	NULL	decomposition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The employment of evolving factor analysis and multivariate curve resolution-alternating least squares for decomposition of the series of quantum dots fluorescence spectra recorded by a specific measuring procedure reveals the number of quantum dot fractions having different diameters .
	manualset3
149270	5	409849	7	NULL	NULL	0	NULL	series of quantum dots fluorescence spectra	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The employment of evolving factor analysis and multivariate curve resolution-alternating least squares for decomposition of the series of quantum dots fluorescence spectra recorded by a specific measuring procedure reveals the number of quantum dot fractions having different diameters .
	manualset3
149271	6	409849	7	NULL	NULL	NULL	NULL	specific measuring procedure	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The employment of evolving factor analysis and multivariate curve resolution-alternating least squares for decomposition of the series of quantum dots fluorescence spectra recorded by a specific measuring procedure reveals the number of quantum dot fractions having different diameters .
	manualset3
149272	7	409849	7	NULL	NULL	NULL	NULL	number of quantum dot fractions	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The employment of evolving factor analysis and multivariate curve resolution-alternating least squares for decomposition of the series of quantum dots fluorescence spectra recorded by a specific measuring procedure reveals the number of quantum dot fractions having different diameters .
	manualset3
149273	8	409849	7	NULL	NULL	NULL	NULL	different diameters	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The employment of evolving factor analysis and multivariate curve resolution-alternating least squares for decomposition of the series of quantum dots fluorescence spectra recorded by a specific measuring procedure reveals the number of quantum dot fractions having different diameters .
	manualset3
149274	1	409850	7	NULL	NULL	0	NULL	enantiomers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The enantiomers of its metabolite 3 , 4-methylenedioxyamphetamine ( MDA ) were also quantified in most hair segments .
	manualset3
149275	2	409850	7	NULL	NULL	0	NULL	 metabolite 3 , 4-methylenedioxyamphetamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The enantiomers of its metabolite 3 , 4-methylenedioxyamphetamine ( MDA ) were also quantified in most hair segments .
	manualset3
149276	3	409850	7	NULL	NULL	0	NULL	hair segments	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The enantiomers of its metabolite 3 , 4-methylenedioxyamphetamine ( MDA ) were also quantified in most hair segments .
	manualset3
149633	1	409851	7	NULL	NULL	0	NULL	encapsulated cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The encapsulated cells ' morphology and roughness characteristics remained intact over a substantial storage period .
	manualset3
149676	2	409851	7	NULL	NULL	0	NULL	morphology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The encapsulated cells ' morphology and roughness characteristics remained intact over a substantial storage period .
	manualset3
149677	3	409851	7	NULL	NULL	0	NULL	roughness	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The encapsulated cells ' morphology and roughness characteristics remained intact over a substantial storage period .
	manualset3
149678	4	409851	7	NULL	NULL	0	NULL	substantial storage period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The encapsulated cells ' morphology and roughness characteristics remained intact over a substantial storage period .
	manualset3
149679	1	409852	7	NULL	NULL	0	NULL	end-point 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The end-point chosen was the inhibition of incidence and growth of putative preneoplastic lesions , the aberrant crypt foci ( ACF ) induced in the rat colon by two administrations of 1 , 2-dimethylhydrazine ( DMH , 25 mg/kg p.o. ) .
	manualset3
149680	2	409852	7	NULL	NULL	0	NULL	 inhibition of incidence	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The end-point chosen was the inhibition of incidence and growth of putative preneoplastic lesions , the aberrant crypt foci ( ACF ) induced in the rat colon by two administrations of 1 , 2-dimethylhydrazine ( DMH , 25 mg/kg p.o. ) .
	manualset3
149681	3	409852	7	NULL	NULL	0	NULL	growth of putative preneoplastic lesions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The end-point chosen was the inhibition of incidence and growth of putative preneoplastic lesions , the aberrant crypt foci ( ACF ) induced in the rat colon by two administrations of 1 , 2-dimethylhydrazine ( DMH , 25 mg/kg p.o. ) .
	manualset3
149682	4	409852	7	NULL	NULL	0	NULL	aberrant crypt foci ( ACF )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The end-point chosen was the inhibition of incidence and growth of putative preneoplastic lesions , the aberrant crypt foci ( ACF ) induced in the rat colon by two administrations of 1 , 2-dimethylhydrazine ( DMH , 25 mg/kg p.o. ) .
	manualset3
149683	5	409852	7	NULL	NULL	0	NULL	 rat colon	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The end-point chosen was the inhibition of incidence and growth of putative preneoplastic lesions , the aberrant crypt foci ( ACF ) induced in the rat colon by two administrations of 1 , 2-dimethylhydrazine ( DMH , 25 mg/kg p.o. ) .
	manualset3
149684	7	409852	7	NULL	NULL	NULL	NULL	1 , 2-dimethylhydrazine DMH	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The end-point chosen was the inhibition of incidence and growth of putative preneoplastic lesions , the aberrant crypt foci ( ACF ) induced in the rat colon by two administrations of 1 , 2-dimethylhydrazine ( DMH , 25 mg/kg p.o. ) .
	manualset3
149685	8	409852	7	NULL	NULL	NULL	NULL	25 mg/kg p.o. 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The end-point chosen was the inhibition of incidence and growth of putative preneoplastic lesions , the aberrant crypt foci ( ACF ) induced in the rat colon by two administrations of 1 , 2-dimethylhydrazine ( DMH , 25 mg/kg p.o. ) .
	manualset3
149847	6	409852	7	NULL	NULL	0	NULL	administrations 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The end-point chosen was the inhibition of incidence and growth of putative preneoplastic lesions , the aberrant crypt foci ( ACF ) induced in the rat colon by two administrations of 1 , 2-dimethylhydrazine ( DMH , 25 mg/kg p.o. ) .
	manualset3
149686	1	409853	7	NULL	NULL	NULL	NULL	end of the leader sequence	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The end of the leader sequence ( 3 ' CUAAAA , which precedes gs1 ) could also be used for gene2 expression , but this sequence was considerably less efficient .
	manualset3
149687	2	409853	7	NULL	NULL	0	NULL	 3 ' CUAAAA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The end of the leader sequence ( 3 ' CUAAAA , which precedes gs1 ) could also be used for gene2 expression , but this sequence was considerably less efficient .
	manualset3
149688	3	409853	7	NULL	NULL	0	NULL	gs1	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The end of the leader sequence ( 3 ' CUAAAA , which precedes gs1 ) could also be used for gene2 expression , but this sequence was considerably less efficient .
	manualset3
149689	4	409853	7	NULL	NULL	NULL	NULL	gene2  expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The end of the leader sequence ( 3 ' CUAAAA , which precedes gs1 ) could also be used for gene2 expression , but this sequence was considerably less efficient .
	manualset3
149691	5	409853	7	NULL	NULL	NULL	NULL	 sequence	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The end of the leader sequence ( 3 ' CUAAAA , which precedes gs1 ) could also be used for gene2 expression , but this sequence was considerably less efficient .
	manualset3
149692	1	409854	7	NULL	NULL	0	NULL	endocurietherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The endocurietherapy does not require surgery , general or local anesthesia .
	manualset3
149693	2	409854	7	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The endocurietherapy does not require surgery , general or local anesthesia .
	manualset3
149694	3	409854	7	NULL	NULL	NULL	NULL	general anesthesia	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The endocurietherapy does not require surgery , general or local anesthesia .
	manualset3
149695	4	409854	7	NULL	NULL	NULL	NULL	local anesthesia	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The endocurietherapy does not require surgery , general or local anesthesia .
	manualset3
149696	1	409855	7	NULL	NULL	0	NULL	endogenous dopamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The endogenous dopamine content of the cells was determined by high performance liquid chromatography utilizing electrochemical detection .
	manualset3
149697	2	409855	7	NULL	NULL	0	NULL	content of the cells	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The endogenous dopamine content of the cells was determined by high performance liquid chromatography utilizing electrochemical detection .
	manualset3
149698	3	409855	7	NULL	NULL	NULL	NULL	high performance liquid chromatography	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The endogenous dopamine content of the cells was determined by high performance liquid chromatography utilizing electrochemical detection .
	manualset3
149699	4	409855	7	NULL	NULL	NULL	NULL	 electrochemical detection	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The endogenous dopamine content of the cells was determined by high performance liquid chromatography utilizing electrochemical detection .
	manualset3
149700	1	409856	7	NULL	NULL	NULL	NULL	endothelins	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The endothelins and sarafotoxins are two structurally related families of potent vasoactive peptides .
	manualset3
149701	2	409856	7	NULL	NULL	NULL	NULL	sarafotoxins	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The endothelins and sarafotoxins are two structurally related families of potent vasoactive peptides .
	manualset3
149702	3	409856	7	NULL	NULL	NULL	NULL	structurally related families	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The endothelins and sarafotoxins are two structurally related families of potent vasoactive peptides .
	manualset3
149703	4	409856	7	NULL	NULL	NULL	NULL	potent vasoactive peptides	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The endothelins and sarafotoxins are two structurally related families of potent vasoactive peptides .
	manualset3
149704	1	409857	7	NULL	NULL	NULL	NULL	endothelium	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The endothelium is of continuous type and has a large population of plasmalemmal vesicles ; the cells are linked together by tight junctions .
	manualset3
149705	3	409857	7	NULL	NULL	NULL	NULL	large population	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The endothelium is of continuous type and has a large population of plasmalemmal vesicles ; the cells are linked together by tight junctions .
	manualset3
149706	4	409857	7	NULL	NULL	NULL	NULL	plasmalemmal vesicles	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The endothelium is of continuous type and has a large population of plasmalemmal vesicles ; the cells are linked together by tight junctions .
	manualset3
149707	5	409857	7	NULL	NULL	NULL	NULL	cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The endothelium is of continuous type and has a large population of plasmalemmal vesicles ; the cells are linked together by tight junctions .
	manualset3
149708	6	409857	7	NULL	NULL	NULL	NULL	tight junctions	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The endothelium is of continuous type and has a large population of plasmalemmal vesicles ; the cells are linked together by tight junctions .
	manualset3
149709	2	409857	7	NULL	NULL	0	NULL	continuous type	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The endothelium is of continuous type and has a large population of plasmalemmal vesicles ; the cells are linked together by tight junctions .
	manualset3
149710	1	409858	7	NULL	NULL	0	NULL	Cirrhotic cardiomyopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cirrhotic cardiomyopathy : increased circulating pro-brain natriuretic peptide and brain natriuretic peptide in cirrhosis ) .
	manualset3
149711	2	409858	7	NULL	NULL	NULL	NULL	increased circulating pro-brain natriuretic peptide	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Cirrhotic cardiomyopathy : increased circulating pro-brain natriuretic peptide and brain natriuretic peptide in cirrhosis ) .
	manualset3
149712	3	409858	7	NULL	NULL	NULL	NULL	increased brain natriuretic peptide 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Cirrhotic cardiomyopathy : increased circulating pro-brain natriuretic peptide and brain natriuretic peptide in cirrhosis ) .
	manualset3
149713	4	409858	7	NULL	NULL	0	NULL	cirrhosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cirrhotic cardiomyopathy : increased circulating pro-brain natriuretic peptide and brain natriuretic peptide in cirrhosis ) .
	manualset3
149714	1	409859	7	NULL	NULL	NULL	NULL	endothelium	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The endothelium synthesizes a very thick basement membrane ( Descemet 's membrane ) .
	manualset3
149716	2	409859	7	NULL	NULL	NULL	NULL	very thick basement membrane 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The endothelium synthesizes a very thick basement membrane ( Descemet 's membrane ) .
	manualset3
149717	3	409859	7	NULL	NULL	NULL	NULL	Descemet 's membrane	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The endothelium synthesizes a very thick basement membrane ( Descemet 's membrane ) .
	manualset3
149718	1	409860	7	NULL	NULL	0	NULL	energy gap	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The energy gap of the BN sheet narrows due to the strong hybridization between O and BN electronic states when the O locates above a BN bond or a nitrogen atom .
	manualset3
149719	2	409860	7	NULL	NULL	NULL	NULL	BN sheet	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The energy gap of the BN sheet narrows due to the strong hybridization between O and BN electronic states when the O locates above a BN bond or a nitrogen atom .
	manualset3
149720	3	409860	7	NULL	NULL	0	NULL	strong hybridization 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The energy gap of the BN sheet narrows due to the strong hybridization between O and BN electronic states when the O locates above a BN bond or a nitrogen atom .
	manualset3
149721	4	409860	7	NULL	NULL	NULL	NULL	O electronic state	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The energy gap of the BN sheet narrows due to the strong hybridization between O and BN electronic states when the O locates above a BN bond or a nitrogen atom .
	manualset3
149722	5	409860	7	NULL	NULL	NULL	NULL	BN electronic state	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The energy gap of the BN sheet narrows due to the strong hybridization between O and BN electronic states when the O locates above a BN bond or a nitrogen atom .
	manualset3
149723	6	409860	7	NULL	NULL	0	NULL	O	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The energy gap of the BN sheet narrows due to the strong hybridization between O and BN electronic states when the O locates above a BN bond or a nitrogen atom .
	manualset3
149724	7	409860	7	NULL	NULL	NULL	NULL	BN bond	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The energy gap of the BN sheet narrows due to the strong hybridization between O and BN electronic states when the O locates above a BN bond or a nitrogen atom .
	manualset3
149725	8	409860	7	NULL	NULL	0	NULL	nitrogen atom	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The energy gap of the BN sheet narrows due to the strong hybridization between O and BN electronic states when the O locates above a BN bond or a nitrogen atom .
	manualset3
149870	1	409861	7	NULL	NULL	0	NULL	engineered disruption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The engineered disruption of subunit contacts at monoTIM causes movement of the essential side chains of Lys-13 and His-95 away from the catalytic active positions .
	manualset3
149871	2	409861	7	NULL	NULL	NULL	NULL	subunit contacts	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The engineered disruption of subunit contacts at monoTIM causes movement of the essential side chains of Lys-13 and His-95 away from the catalytic active positions .
	manualset3
149872	3	409861	7	NULL	NULL	NULL	NULL	monoTIM	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The engineered disruption of subunit contacts at monoTIM causes movement of the essential side chains of Lys-13 and His-95 away from the catalytic active positions .
	manualset3
149873	4	409861	7	NULL	NULL	0	NULL	 movement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The engineered disruption of subunit contacts at monoTIM causes movement of the essential side chains of Lys-13 and His-95 away from the catalytic active positions .
	manualset3
149874	5	409861	7	NULL	NULL	0	NULL	essential side chains of Lys-13	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The engineered disruption of subunit contacts at monoTIM causes movement of the essential side chains of Lys-13 and His-95 away from the catalytic active positions .
	manualset3
149875	6	409861	7	NULL	NULL	0	NULL	essential side chains of His-95	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The engineered disruption of subunit contacts at monoTIM causes movement of the essential side chains of Lys-13 and His-95 away from the catalytic active positions .
	manualset3
149876	7	409861	7	NULL	NULL	NULL	NULL	catalytic active positions	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The engineered disruption of subunit contacts at monoTIM causes movement of the essential side chains of Lys-13 and His-95 away from the catalytic active positions .
	manualset3
149877	1	409862	7	NULL	NULL	NULL	NULL	enhancing effects 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enhancing effects of TNF-alpha and PDGF-BB were attenuated by PD98059 ( an inhibitor of activation of MAPK kinase , MEK ) and cycloheximide ( an inhibitor of protein synthesis ) , suggesting that TNF-alpha may share a common signalling pathway with PDGF-BB via protein ( s ) synthesis in TSMCs .
	manualset3
149878	2	409862	7	NULL	NULL	0	NULL	TNF-alpha 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enhancing effects of TNF-alpha and PDGF-BB were attenuated by PD98059 ( an inhibitor of activation of MAPK kinase , MEK ) and cycloheximide ( an inhibitor of protein synthesis ) , suggesting that TNF-alpha may share a common signalling pathway with PDGF-BB via protein ( s ) synthesis in TSMCs .
	manualset3
149879	3	409862	7	NULL	NULL	0	NULL	PDGF-BB	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enhancing effects of TNF-alpha and PDGF-BB were attenuated by PD98059 ( an inhibitor of activation of MAPK kinase , MEK ) and cycloheximide ( an inhibitor of protein synthesis ) , suggesting that TNF-alpha may share a common signalling pathway with PDGF-BB via protein ( s ) synthesis in TSMCs .
	manualset3
149880	4	409862	7	NULL	NULL	0	NULL	PD98059	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The enhancing effects of TNF-alpha and PDGF-BB were attenuated by PD98059 ( an inhibitor of activation of MAPK kinase , MEK ) and cycloheximide ( an inhibitor of protein synthesis ) , suggesting that TNF-alpha may share a common signalling pathway with PDGF-BB via protein ( s ) synthesis in TSMCs .
	manualset3
149881	6	409862	7	NULL	NULL	NULL	NULL	activation of MAPK kinase	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enhancing effects of TNF-alpha and PDGF-BB were attenuated by PD98059 ( an inhibitor of activation of MAPK kinase , MEK ) and cycloheximide ( an inhibitor of protein synthesis ) , suggesting that TNF-alpha may share a common signalling pathway with PDGF-BB via protein ( s ) synthesis in TSMCs .
	manualset3
149883	8	409862	7	NULL	NULL	NULL	NULL	cycloheximide	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enhancing effects of TNF-alpha and PDGF-BB were attenuated by PD98059 ( an inhibitor of activation of MAPK kinase , MEK ) and cycloheximide ( an inhibitor of protein synthesis ) , suggesting that TNF-alpha may share a common signalling pathway with PDGF-BB via protein ( s ) synthesis in TSMCs .
	manualset3
149886	9	409862	7	NULL	NULL	NULL	NULL	inhibitor	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enhancing effects of TNF-alpha and PDGF-BB were attenuated by PD98059 ( an inhibitor of activation of MAPK kinase , MEK ) and cycloheximide ( an inhibitor of protein synthesis ) , suggesting that TNF-alpha may share a common signalling pathway with PDGF-BB via protein ( s ) synthesis in TSMCs .
	manualset3
149889	11	409862	7	NULL	NULL	NULL	NULL	TNF-alpha	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enhancing effects of TNF-alpha and PDGF-BB were attenuated by PD98059 ( an inhibitor of activation of MAPK kinase , MEK ) and cycloheximide ( an inhibitor of protein synthesis ) , suggesting that TNF-alpha may share a common signalling pathway with PDGF-BB via protein ( s ) synthesis in TSMCs .
	manualset3
149891	12	409862	7	NULL	NULL	NULL	NULL	common signalling pathway	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enhancing effects of TNF-alpha and PDGF-BB were attenuated by PD98059 ( an inhibitor of activation of MAPK kinase , MEK ) and cycloheximide ( an inhibitor of protein synthesis ) , suggesting that TNF-alpha may share a common signalling pathway with PDGF-BB via protein ( s ) synthesis in TSMCs .
	manualset3
149895	13	409862	7	NULL	NULL	NULL	NULL	PDGF-BB	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enhancing effects of TNF-alpha and PDGF-BB were attenuated by PD98059 ( an inhibitor of activation of MAPK kinase , MEK ) and cycloheximide ( an inhibitor of protein synthesis ) , suggesting that TNF-alpha may share a common signalling pathway with PDGF-BB via protein ( s ) synthesis in TSMCs .
	manualset3
149896	14	409862	7	NULL	NULL	NULL	NULL	protein ( s ) synthesis	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enhancing effects of TNF-alpha and PDGF-BB were attenuated by PD98059 ( an inhibitor of activation of MAPK kinase , MEK ) and cycloheximide ( an inhibitor of protein synthesis ) , suggesting that TNF-alpha may share a common signalling pathway with PDGF-BB via protein ( s ) synthesis in TSMCs .
	manualset3
149897	15	409862	7	NULL	NULL	NULL	NULL	TSMCs	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enhancing effects of TNF-alpha and PDGF-BB were attenuated by PD98059 ( an inhibitor of activation of MAPK kinase , MEK ) and cycloheximide ( an inhibitor of protein synthesis ) , suggesting that TNF-alpha may share a common signalling pathway with PDGF-BB via protein ( s ) synthesis in TSMCs .
	manualset3
150095	5	409862	7	NULL	NULL	NULL	NULL	inhibitor 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enhancing effects of TNF-alpha and PDGF-BB were attenuated by PD98059 ( an inhibitor of activation of MAPK kinase , MEK ) and cycloheximide ( an inhibitor of protein synthesis ) , suggesting that TNF-alpha may share a common signalling pathway with PDGF-BB via protein ( s ) synthesis in TSMCs .
	manualset3
150096	7	409862	7	NULL	NULL	NULL	NULL	MEK	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enhancing effects of TNF-alpha and PDGF-BB were attenuated by PD98059 ( an inhibitor of activation of MAPK kinase , MEK ) and cycloheximide ( an inhibitor of protein synthesis ) , suggesting that TNF-alpha may share a common signalling pathway with PDGF-BB via protein ( s ) synthesis in TSMCs .
	manualset3
150097	10	409862	7	NULL	NULL	NULL	NULL	protein synthesis	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enhancing effects of TNF-alpha and PDGF-BB were attenuated by PD98059 ( an inhibitor of activation of MAPK kinase , MEK ) and cycloheximide ( an inhibitor of protein synthesis ) , suggesting that TNF-alpha may share a common signalling pathway with PDGF-BB via protein ( s ) synthesis in TSMCs .
	manualset3
149916	1	409863	7	NULL	NULL	0	NULL	enriched metabolite profile	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The enriched metabolite profile , particularly in the cortical areas , is consistent with the hypothesis that decreased glucose use in the traumatized brain is caused by diminished need rather than by decreased supply of energy .
	manualset3
149917	2	409863	7	NULL	NULL	0	NULL	cortical areas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The enriched metabolite profile , particularly in the cortical areas , is consistent with the hypothesis that decreased glucose use in the traumatized brain is caused by diminished need rather than by decreased supply of energy .
	manualset3
149918	3	409863	7	NULL	NULL	NULL	NULL	 hypothesis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enriched metabolite profile , particularly in the cortical areas , is consistent with the hypothesis that decreased glucose use in the traumatized brain is caused by diminished need rather than by decreased supply of energy .
	manualset3
149919	4	409863	7	NULL	NULL	NULL	NULL	decreased glucose use	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enriched metabolite profile , particularly in the cortical areas , is consistent with the hypothesis that decreased glucose use in the traumatized brain is caused by diminished need rather than by decreased supply of energy .
	manualset3
149920	5	409863	7	NULL	NULL	0	NULL	traumatized brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The enriched metabolite profile , particularly in the cortical areas , is consistent with the hypothesis that decreased glucose use in the traumatized brain is caused by diminished need rather than by decreased supply of energy .
	manualset3
149921	6	409863	7	NULL	NULL	NULL	NULL	diminished need	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enriched metabolite profile , particularly in the cortical areas , is consistent with the hypothesis that decreased glucose use in the traumatized brain is caused by diminished need rather than by decreased supply of energy .
	manualset3
149922	7	409863	7	NULL	NULL	NULL	NULL	decreased supply of energy	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enriched metabolite profile , particularly in the cortical areas , is consistent with the hypothesis that decreased glucose use in the traumatized brain is caused by diminished need rather than by decreased supply of energy .
	manualset3
149923	1	409864	7	NULL	NULL	NULL	NULL	entry 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The entry of calcium ions into cells through voltage-activated Ca2 + channels in the plasma membrane triggers many important cellular processes .
	manualset3
149924	3	409864	7	NULL	NULL	NULL	NULL	cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The entry of calcium ions into cells through voltage-activated Ca2 + channels in the plasma membrane triggers many important cellular processes .
	manualset3
149925	4	409864	7	NULL	NULL	NULL	NULL	voltage-activated Ca2 + channels	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The entry of calcium ions into cells through voltage-activated Ca2 + channels in the plasma membrane triggers many important cellular processes .
	manualset3
149926	5	409864	7	NULL	NULL	NULL	NULL	plasma membrane	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The entry of calcium ions into cells through voltage-activated Ca2 + channels in the plasma membrane triggers many important cellular processes .
	manualset3
149927	6	409864	7	NULL	NULL	NULL	NULL	important cellular processes	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The entry of calcium ions into cells through voltage-activated Ca2 + channels in the plasma membrane triggers many important cellular processes .
	manualset3
150192	2	409864	7	NULL	NULL	0	NULL	calcium ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The entry of calcium ions into cells through voltage-activated Ca2 + channels in the plasma membrane triggers many important cellular processes .
	manualset3
149928	1	409865	7	NULL	NULL	0	NULL	environment	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The environment has a teacher mode and a student mode .
	manualset3
149929	2	409865	7	NULL	NULL	NULL	NULL	teacher mode	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The environment has a teacher mode and a student mode .
	manualset3
149930	3	409865	7	NULL	NULL	NULL	NULL	student mode	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The environment has a teacher mode and a student mode .
	manualset3
149939	1	409866	7	NULL	NULL	0	NULL	enzymatic activities 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzymatic activities were partially characterized from both adult worm species and demonstrated a preference for ( 3H ) GPI substrate over ( 3H ) PI .
	manualset3
149940	2	409866	7	NULL	NULL	NULL	NULL	adult worm species	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzymatic activities were partially characterized from both adult worm species and demonstrated a preference for ( 3H ) GPI substrate over ( 3H ) PI .
	manualset3
149942	3	409866	7	NULL	NULL	NULL	NULL	( 3H ) GPI	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzymatic activities were partially characterized from both adult worm species and demonstrated a preference for ( 3H ) GPI substrate over ( 3H ) PI .
	manualset3
149943	4	409866	7	NULL	NULL	NULL	NULL	( 3H ) PI 	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzymatic activities were partially characterized from both adult worm species and demonstrated a preference for ( 3H ) GPI substrate over ( 3H ) PI .
	manualset3
149944	1	409867	7	NULL	NULL	0	NULL	enzyme-linked immunosorbent assay ( ELISA )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme-linked immunosorbent assay ( ELISA ) has been used to study the serum IgM and IgG response and the bile IgA and IgM response of chickens to a primary , secondary and tertiary inoculation of Eimeria tenella .
	manualset3
149946	2	409867	7	NULL	NULL	NULL	NULL	serum IgM response	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme-linked immunosorbent assay ( ELISA ) has been used to study the serum IgM and IgG response and the bile IgA and IgM response of chickens to a primary , secondary and tertiary inoculation of Eimeria tenella .
	manualset3
149947	3	409867	7	NULL	NULL	NULL	NULL	serum IgG response	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme-linked immunosorbent assay ( ELISA ) has been used to study the serum IgM and IgG response and the bile IgA and IgM response of chickens to a primary , secondary and tertiary inoculation of Eimeria tenella .
	manualset3
149948	4	409867	7	NULL	NULL	NULL	NULL	bile IgA response	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme-linked immunosorbent assay ( ELISA ) has been used to study the serum IgM and IgG response and the bile IgA and IgM response of chickens to a primary , secondary and tertiary inoculation of Eimeria tenella .
	manualset3
149949	5	409867	7	NULL	NULL	NULL	NULL	bile IgM response 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme-linked immunosorbent assay ( ELISA ) has been used to study the serum IgM and IgG response and the bile IgA and IgM response of chickens to a primary , secondary and tertiary inoculation of Eimeria tenella .
	manualset3
149950	6	409867	7	NULL	NULL	NULL	NULL	chickens	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme-linked immunosorbent assay ( ELISA ) has been used to study the serum IgM and IgG response and the bile IgA and IgM response of chickens to a primary , secondary and tertiary inoculation of Eimeria tenella .
	manualset3
149951	7	409867	7	NULL	NULL	NULL	NULL	primary inoculation 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme-linked immunosorbent assay ( ELISA ) has been used to study the serum IgM and IgG response and the bile IgA and IgM response of chickens to a primary , secondary and tertiary inoculation of Eimeria tenella .
	manualset3
149952	8	409867	7	NULL	NULL	NULL	NULL	secondary inoculation 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme-linked immunosorbent assay ( ELISA ) has been used to study the serum IgM and IgG response and the bile IgA and IgM response of chickens to a primary , secondary and tertiary inoculation of Eimeria tenella .
	manualset3
149953	9	409867	7	NULL	NULL	NULL	NULL	tertiary inoculation 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme-linked immunosorbent assay ( ELISA ) has been used to study the serum IgM and IgG response and the bile IgA and IgM response of chickens to a primary , secondary and tertiary inoculation of Eimeria tenella .
	manualset3
150093	10	409867	7	NULL	NULL	NULL	NULL	Eimeria tenella	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme-linked immunosorbent assay ( ELISA ) has been used to study the serum IgM and IgG response and the bile IgA and IgM response of chickens to a primary , secondary and tertiary inoculation of Eimeria tenella .
	manualset3
149954	1	409868	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A study of delayed hypersensitivity of guinea pigs to vaccinia virus .
	manualset3
149955	2	409868	7	NULL	NULL	0	NULL	delayed hypersensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A study of delayed hypersensitivity of guinea pigs to vaccinia virus .
	manualset3
149956	3	409868	7	NULL	NULL	0	NULL	guinea pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A study of delayed hypersensitivity of guinea pigs to vaccinia virus .
	manualset3
149957	4	409868	7	NULL	NULL	0	NULL	vaccinia virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A study of delayed hypersensitivity of guinea pigs to vaccinia virus .
	manualset3
149958	1	409869	7	NULL	NULL	0	NULL	enzyme activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme activity peaked during a 28-h observation period .
	manualset3
149959	2	409869	7	NULL	NULL	0	NULL	28-h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme activity peaked during a 28-h observation period .
	manualset3
149960	3	409869	7	NULL	NULL	0	NULL	observation period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme activity peaked during a 28-h observation period .
	manualset3
149961	1	409870	7	NULL	NULL	NULL	NULL	enzyme blank	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme blank and boiled enzyme blank failed to show any significant HPLC peaks corresponding to retinal O-ethyloxime , retinal , or retinol .
	manualset3
149962	2	409870	7	NULL	NULL	NULL	NULL	boiled enzyme blank	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme blank and boiled enzyme blank failed to show any significant HPLC peaks corresponding to retinal O-ethyloxime , retinal , or retinol .
	manualset3
149964	3	409870	7	NULL	NULL	NULL	NULL	significant HPLC peaks 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme blank and boiled enzyme blank failed to show any significant HPLC peaks corresponding to retinal O-ethyloxime , retinal , or retinol .
	manualset3
149965	4	409870	7	NULL	NULL	NULL	NULL	retinal O-ethyloxime	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme blank and boiled enzyme blank failed to show any significant HPLC peaks corresponding to retinal O-ethyloxime , retinal , or retinol .
	manualset3
149966	5	409870	7	NULL	NULL	NULL	NULL	retinal 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme blank and boiled enzyme blank failed to show any significant HPLC peaks corresponding to retinal O-ethyloxime , retinal , or retinol .
	manualset3
149967	6	409870	7	NULL	NULL	NULL	NULL	 retinol	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme blank and boiled enzyme blank failed to show any significant HPLC peaks corresponding to retinal O-ethyloxime , retinal , or retinol .
	manualset3
149968	1	409871	7	NULL	NULL	0	NULL	enzyme carnitine palmitoyltransferase 1 ( CPT1 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme carnitine palmitoyltransferase 1 ( CPT1 ) , which is anchored in the outer mitochondrial membrane ( OMM ) , controls the rate-limiting step in fatty acid - oxidation in mammalian tissues .
	manualset3
149970	2	409871	7	NULL	NULL	NULL	NULL	outer mitochondrial membrane ( OMM )	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme carnitine palmitoyltransferase 1 ( CPT1 ) , which is anchored in the outer mitochondrial membrane ( OMM ) , controls the rate-limiting step in fatty acid - oxidation in mammalian tissues .
	manualset3
149971	3	409871	7	NULL	NULL	NULL	NULL	rate-limiting step	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme carnitine palmitoyltransferase 1 ( CPT1 ) , which is anchored in the outer mitochondrial membrane ( OMM ) , controls the rate-limiting step in fatty acid - oxidation in mammalian tissues .
	manualset3
149972	4	409871	7	NULL	NULL	NULL	NULL	 fatty acid - oxidation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme carnitine palmitoyltransferase 1 ( CPT1 ) , which is anchored in the outer mitochondrial membrane ( OMM ) , controls the rate-limiting step in fatty acid - oxidation in mammalian tissues .
	manualset3
149973	5	409871	7	NULL	NULL	NULL	NULL	mammalian tissues	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme carnitine palmitoyltransferase 1 ( CPT1 ) , which is anchored in the outer mitochondrial membrane ( OMM ) , controls the rate-limiting step in fatty acid - oxidation in mammalian tissues .
	manualset3
149974	1	409872	7	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme contains one atom of Zn per molecule , is activated by Ca2 + and is drastically inhibited by the metal chelator 1 , 10-phenanthroline , as well as by excess Zn2 + or Cu2 + , but moderately so by EDTA .
	manualset3
149975	2	409872	7	NULL	NULL	NULL	NULL	atom of Zn per molecule	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme contains one atom of Zn per molecule , is activated by Ca2 + and is drastically inhibited by the metal chelator 1 , 10-phenanthroline , as well as by excess Zn2 + or Cu2 + , but moderately so by EDTA .
	manualset3
149976	3	409872	7	NULL	NULL	0	NULL	Ca2+	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme contains one atom of Zn per molecule , is activated by Ca2 + and is drastically inhibited by the metal chelator 1 , 10-phenanthroline , as well as by excess Zn2 + or Cu2 + , but moderately so by EDTA .
	manualset3
149977	4	409872	7	NULL	NULL	0	NULL	metal chelator 1 , 10-phenanthroline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme contains one atom of Zn per molecule , is activated by Ca2 + and is drastically inhibited by the metal chelator 1 , 10-phenanthroline , as well as by excess Zn2 + or Cu2 + , but moderately so by EDTA .
	manualset3
149978	5	409872	7	NULL	NULL	0	NULL	excess Zn2 +	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme contains one atom of Zn per molecule , is activated by Ca2 + and is drastically inhibited by the metal chelator 1 , 10-phenanthroline , as well as by excess Zn2 + or Cu2 + , but moderately so by EDTA .
	manualset3
149979	6	409872	7	NULL	NULL	0	NULL	excess Cu2+	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme contains one atom of Zn per molecule , is activated by Ca2 + and is drastically inhibited by the metal chelator 1 , 10-phenanthroline , as well as by excess Zn2 + or Cu2 + , but moderately so by EDTA .
	manualset3
149980	7	409872	7	NULL	NULL	0	NULL	EDTA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme contains one atom of Zn per molecule , is activated by Ca2 + and is drastically inhibited by the metal chelator 1 , 10-phenanthroline , as well as by excess Zn2 + or Cu2 + , but moderately so by EDTA .
	manualset3
149981	1	409873	7	NULL	NULL	0	NULL	 enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme folds into two distinct domains : a catalytic beta-propeller fold tightly associated with a lectin-like domain .
	manualset3
149982	2	409873	7	NULL	NULL	NULL	NULL	two distinct domains	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme folds into two distinct domains : a catalytic beta-propeller fold tightly associated with a lectin-like domain .
	manualset3
149983	3	409873	7	NULL	NULL	0	NULL	catalytic beta-propeller fold	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme folds into two distinct domains : a catalytic beta-propeller fold tightly associated with a lectin-like domain .
	manualset3
149984	4	409873	7	NULL	NULL	0	NULL	 lectin-like domain 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme folds into two distinct domains : a catalytic beta-propeller fold tightly associated with a lectin-like domain .
	manualset3
149985	1	409874	7	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme has a pH optimum of 6.5 for the reduction of L-lactaldehyde and of 9.5 for the dehydrogenation of L-1 , 2 - propanediol .
	manualset3
149986	2	409874	7	NULL	NULL	NULL	NULL	pH optimum	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme has a pH optimum of 6.5 for the reduction of L-lactaldehyde and of 9.5 for the dehydrogenation of L-1 , 2 - propanediol .
	manualset3
149987	3	409874	7	NULL	NULL	NULL	NULL	6.5	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme has a pH optimum of 6.5 for the reduction of L-lactaldehyde and of 9.5 for the dehydrogenation of L-1 , 2 - propanediol .
	manualset3
149988	5	409874	7	NULL	NULL	NULL	NULL	L-lactaldehyde	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme has a pH optimum of 6.5 for the reduction of L-lactaldehyde and of 9.5 for the dehydrogenation of L-1 , 2 - propanediol .
	manualset3
149989	6	409874	7	NULL	NULL	NULL	NULL	9.5	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme has a pH optimum of 6.5 for the reduction of L-lactaldehyde and of 9.5 for the dehydrogenation of L-1 , 2 - propanediol .
	manualset3
149990	7	409874	7	NULL	NULL	NULL	NULL	dehydrogenation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme has a pH optimum of 6.5 for the reduction of L-lactaldehyde and of 9.5 for the dehydrogenation of L-1 , 2 - propanediol .
	manualset3
149991	8	409874	7	NULL	NULL	NULL	NULL	L-1 , 2 - propanediol	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme has a pH optimum of 6.5 for the reduction of L-lactaldehyde and of 9.5 for the dehydrogenation of L-1 , 2 - propanediol .
	manualset3
149992	4	409874	7	NULL	NULL	0	NULL	reduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme has a pH optimum of 6.5 for the reduction of L-lactaldehyde and of 9.5 for the dehydrogenation of L-1 , 2 - propanediol .
	manualset3
149993	1	409875	7	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme has no transamidation activity with L-alanyl amide both as aminoacyl donator and - acceptor .
	manualset3
149994	2	409875	7	NULL	NULL	NULL	NULL	 transamidation activity 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme has no transamidation activity with L-alanyl amide both as aminoacyl donator and - acceptor .
	manualset3
149995	3	409875	7	NULL	NULL	0	NULL	L-alanyl amide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme has no transamidation activity with L-alanyl amide both as aminoacyl donator and - acceptor .
	manualset3
149996	4	409875	7	NULL	NULL	0	NULL	aminoacyl donator	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme has no transamidation activity with L-alanyl amide both as aminoacyl donator and - acceptor .
	manualset3
149997	5	409875	7	NULL	NULL	0	NULL	aminoacyl - acceptor	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme has no transamidation activity with L-alanyl amide both as aminoacyl donator and - acceptor .
	manualset3
149998	1	409876	7	NULL	NULL	0	NULL	 enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme histochemical and intermediate filament patterns were usually the same as those described previously for proliferative foci and early tumors , i.e. highly elevated activities of glucose-6-phosphate dehydrogenase , adenylate cyclase and alkaline phosphatase , a lack of glucose-6-phosphatase and gamma-glutamyltransferase and coexpression of vimentin and desmin , alpha-smooth muscle actin could not be detected in early lesions .
	manualset3
149999	2	409876	7	NULL	NULL	0	NULL	histochemical and intermediate filament patterns	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme histochemical and intermediate filament patterns were usually the same as those described previously for proliferative foci and early tumors , i.e. highly elevated activities of glucose-6-phosphate dehydrogenase , adenylate cyclase and alkaline phosphatase , a lack of glucose-6-phosphatase and gamma-glutamyltransferase and coexpression of vimentin and desmin , alpha-smooth muscle actin could not be detected in early lesions .
	manualset3
150000	3	409876	7	NULL	NULL	0	NULL	proliferative foci	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme histochemical and intermediate filament patterns were usually the same as those described previously for proliferative foci and early tumors , i.e. highly elevated activities of glucose-6-phosphate dehydrogenase , adenylate cyclase and alkaline phosphatase , a lack of glucose-6-phosphatase and gamma-glutamyltransferase and coexpression of vimentin and desmin , alpha-smooth muscle actin could not be detected in early lesions .
	manualset3
150001	4	409876	7	NULL	NULL	NULL	NULL	early tumors	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme histochemical and intermediate filament patterns were usually the same as those described previously for proliferative foci and early tumors , i.e. highly elevated activities of glucose-6-phosphate dehydrogenase , adenylate cyclase and alkaline phosphatase , a lack of glucose-6-phosphatase and gamma-glutamyltransferase and coexpression of vimentin and desmin , alpha-smooth muscle actin could not be detected in early lesions .
	manualset3
150002	5	409876	7	NULL	NULL	0	NULL	highly elevated activities of glucose-6-phosphate dehydrogenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme histochemical and intermediate filament patterns were usually the same as those described previously for proliferative foci and early tumors , i.e. highly elevated activities of glucose-6-phosphate dehydrogenase , adenylate cyclase and alkaline phosphatase , a lack of glucose-6-phosphatase and gamma-glutamyltransferase and coexpression of vimentin and desmin , alpha-smooth muscle actin could not be detected in early lesions .
	manualset3
150003	6	409876	7	NULL	NULL	0	NULL	highly elevated activities of adenylate cyclase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme histochemical and intermediate filament patterns were usually the same as those described previously for proliferative foci and early tumors , i.e. highly elevated activities of glucose-6-phosphate dehydrogenase , adenylate cyclase and alkaline phosphatase , a lack of glucose-6-phosphatase and gamma-glutamyltransferase and coexpression of vimentin and desmin , alpha-smooth muscle actin could not be detected in early lesions .
	manualset3
150004	7	409876	7	NULL	NULL	0	NULL	highly elevated activities of alkaline phosphatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme histochemical and intermediate filament patterns were usually the same as those described previously for proliferative foci and early tumors , i.e. highly elevated activities of glucose-6-phosphate dehydrogenase , adenylate cyclase and alkaline phosphatase , a lack of glucose-6-phosphatase and gamma-glutamyltransferase and coexpression of vimentin and desmin , alpha-smooth muscle actin could not be detected in early lesions .
	manualset3
150005	8	409876	7	NULL	NULL	0	NULL	lack of glucose-6-phosphatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme histochemical and intermediate filament patterns were usually the same as those described previously for proliferative foci and early tumors , i.e. highly elevated activities of glucose-6-phosphate dehydrogenase , adenylate cyclase and alkaline phosphatase , a lack of glucose-6-phosphatase and gamma-glutamyltransferase and coexpression of vimentin and desmin , alpha-smooth muscle actin could not be detected in early lesions .
	manualset3
150006	9	409876	7	NULL	NULL	0	NULL	lack of gamma-glutamyltransferase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme histochemical and intermediate filament patterns were usually the same as those described previously for proliferative foci and early tumors , i.e. highly elevated activities of glucose-6-phosphate dehydrogenase , adenylate cyclase and alkaline phosphatase , a lack of glucose-6-phosphatase and gamma-glutamyltransferase and coexpression of vimentin and desmin , alpha-smooth muscle actin could not be detected in early lesions .
	manualset3
150007	10	409876	7	NULL	NULL	0	NULL	coexpression of vimentin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme histochemical and intermediate filament patterns were usually the same as those described previously for proliferative foci and early tumors , i.e. highly elevated activities of glucose-6-phosphate dehydrogenase , adenylate cyclase and alkaline phosphatase , a lack of glucose-6-phosphatase and gamma-glutamyltransferase and coexpression of vimentin and desmin , alpha-smooth muscle actin could not be detected in early lesions .
	manualset3
150008	11	409876	7	NULL	NULL	0	NULL	coexpression of desmin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme histochemical and intermediate filament patterns were usually the same as those described previously for proliferative foci and early tumors , i.e. highly elevated activities of glucose-6-phosphate dehydrogenase , adenylate cyclase and alkaline phosphatase , a lack of glucose-6-phosphatase and gamma-glutamyltransferase and coexpression of vimentin and desmin , alpha-smooth muscle actin could not be detected in early lesions .
	manualset3
150009	12	409876	7	NULL	NULL	0	NULL	coexpression of alpha-smooth muscle actin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme histochemical and intermediate filament patterns were usually the same as those described previously for proliferative foci and early tumors , i.e. highly elevated activities of glucose-6-phosphate dehydrogenase , adenylate cyclase and alkaline phosphatase , a lack of glucose-6-phosphatase and gamma-glutamyltransferase and coexpression of vimentin and desmin , alpha-smooth muscle actin could not be detected in early lesions .
	manualset3
150010	13	409876	7	NULL	NULL	0	NULL	early lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme histochemical and intermediate filament patterns were usually the same as those described previously for proliferative foci and early tumors , i.e. highly elevated activities of glucose-6-phosphate dehydrogenase , adenylate cyclase and alkaline phosphatase , a lack of glucose-6-phosphatase and gamma-glutamyltransferase and coexpression of vimentin and desmin , alpha-smooth muscle actin could not be detected in early lesions .
	manualset3
150011	1	409877	7	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme is a dimer of 140 kDa with identical subunits of 75 kDa .
	manualset3
150012	2	409877	7	NULL	NULL	NULL	NULL	dimer 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme is a dimer of 140 kDa with identical subunits of 75 kDa .
	manualset3
150013	4	409877	7	NULL	NULL	NULL	NULL	identical subunits	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme is a dimer of 140 kDa with identical subunits of 75 kDa .
	manualset3
150014	4	409877	7	NULL	NULL	NULL	NULL	75 kDa	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme is a dimer of 140 kDa with identical subunits of 75 kDa .
	manualset3
150094	3	409877	7	NULL	NULL	0	NULL	140kDa	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme is a dimer of 140 kDa with identical subunits of 75 kDa .
	manualset3
150015	1	409878	7	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme is a single polypeptide chain of 216 residues .
	manualset3
150016	2	409878	7	NULL	NULL	0	NULL	single polypeptide chain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme is a single polypeptide chain of 216 residues .
	manualset3
150017	3	409878	7	NULL	NULL	0	NULL	216 residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme is a single polypeptide chain of 216 residues .
	manualset3
150018	1	409879	7	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme is tolerated even in repetitive doses .
	manualset3
150019	2	409879	7	NULL	NULL	NULL	NULL	repetitive doses	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme is tolerated even in repetitive doses .
	manualset3
150020	1	409880	7	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme may be a potential target for therapeutic intervention of colorectal cancers .
	manualset3
150021	2	409880	7	NULL	NULL	0	NULL	potential target	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme may be a potential target for therapeutic intervention of colorectal cancers .
	manualset3
150022	3	409880	7	NULL	NULL	0	NULL	therapeutic intervention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme may be a potential target for therapeutic intervention of colorectal cancers .
	manualset3
150023	4	409880	7	NULL	NULL	NULL	NULL	colorectal cancers	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme may be a potential target for therapeutic intervention of colorectal cancers .
	manualset3
150322	1	409881	7	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme not only phosphorylates dTMP and dUMP but can also tolerate the bulkier purines dGMP , GMP and dIMP .
	manualset3
150324	2	409881	7	NULL	NULL	NULL	NULL	dTMP	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme not only phosphorylates dTMP and dUMP but can also tolerate the bulkier purines dGMP , GMP and dIMP .
	manualset3
150325	4	409881	7	NULL	NULL	NULL	NULL	dUMP	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme not only phosphorylates dTMP and dUMP but can also tolerate the bulkier purines dGMP , GMP and dIMP .
	manualset3
150326	5	409881	7	NULL	NULL	NULL	NULL	bulkier purines dGMP	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme not only phosphorylates dTMP and dUMP but can also tolerate the bulkier purines dGMP , GMP and dIMP .
	manualset3
150327	6	409881	7	NULL	NULL	NULL	NULL	bulkier purines GMP	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme not only phosphorylates dTMP and dUMP but can also tolerate the bulkier purines dGMP , GMP and dIMP .
	manualset3
150328	7	409881	7	NULL	NULL	NULL	NULL	bulkier purines dIMP	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme not only phosphorylates dTMP and dUMP but can also tolerate the bulkier purines dGMP , GMP and dIMP .
	manualset3
150329	1	409882	7	NULL	NULL	0	NULL	 enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme phosphofructokinase-1 ( PFK-1 ) catalyzes the first committed step of glycolysis and is regulated by a complex array of allosteric effectors that integrate glycolytic flux with cellular bioenergetics .
	manualset3
150330	2	409882	7	NULL	NULL	0	NULL	phosphofructokinase-1 ( PFK-1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme phosphofructokinase-1 ( PFK-1 ) catalyzes the first committed step of glycolysis and is regulated by a complex array of allosteric effectors that integrate glycolytic flux with cellular bioenergetics .
	manualset3
150331	3	409882	7	NULL	NULL	0	NULL	committed step	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme phosphofructokinase-1 ( PFK-1 ) catalyzes the first committed step of glycolysis and is regulated by a complex array of allosteric effectors that integrate glycolytic flux with cellular bioenergetics .
	manualset3
150332	4	409882	7	NULL	NULL	0	NULL	glycolysis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme phosphofructokinase-1 ( PFK-1 ) catalyzes the first committed step of glycolysis and is regulated by a complex array of allosteric effectors that integrate glycolytic flux with cellular bioenergetics .
	manualset3
150333	5	409882	7	NULL	NULL	NULL	NULL	complex array of allosteric effectors	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme phosphofructokinase-1 ( PFK-1 ) catalyzes the first committed step of glycolysis and is regulated by a complex array of allosteric effectors that integrate glycolytic flux with cellular bioenergetics .
	manualset3
150334	6	409882	7	NULL	NULL	0	NULL	glycolytic flux	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme phosphofructokinase-1 ( PFK-1 ) catalyzes the first committed step of glycolysis and is regulated by a complex array of allosteric effectors that integrate glycolytic flux with cellular bioenergetics .
	manualset3
150335	7	409882	7	NULL	NULL	0	NULL	cellular bioenergetics	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme phosphofructokinase-1 ( PFK-1 ) catalyzes the first committed step of glycolysis and is regulated by a complex array of allosteric effectors that integrate glycolytic flux with cellular bioenergetics .
	manualset3
150380	1	409883	7	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme was found to be cold labile and extremely unstable in crude hemolysate , with complete loss of activity occurring after 24 hours at 4 degrees C. However , maintenance of crude hemolysate at 20 to 25 degrees C in the presence of EDTA and KCl increased NAD synthetase stability substantially ( half-life = 10 days ) .
	manualset3
150381	2	409883	7	NULL	NULL	0	NULL	cold labile	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme was found to be cold labile and extremely unstable in crude hemolysate , with complete loss of activity occurring after 24 hours at 4 degrees C. However , maintenance of crude hemolysate at 20 to 25 degrees C in the presence of EDTA and KCl increased NAD synthetase stability substantially ( half-life = 10 days ) .
	manualset3
150382	3	409883	7	NULL	NULL	0	NULL	extremely unstable	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme was found to be cold labile and extremely unstable in crude hemolysate , with complete loss of activity occurring after 24 hours at 4 degrees C. However , maintenance of crude hemolysate at 20 to 25 degrees C in the presence of EDTA and KCl increased NAD synthetase stability substantially ( half-life = 10 days ) .
	manualset3
150383	4	409883	7	NULL	NULL	0	NULL	 crude hemolysate	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme was found to be cold labile and extremely unstable in crude hemolysate , with complete loss of activity occurring after 24 hours at 4 degrees C. However , maintenance of crude hemolysate at 20 to 25 degrees C in the presence of EDTA and KCl increased NAD synthetase stability substantially ( half-life = 10 days ) .
	manualset3
150384	5	409883	7	NULL	NULL	0	NULL	complete loss of activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme was found to be cold labile and extremely unstable in crude hemolysate , with complete loss of activity occurring after 24 hours at 4 degrees C. However , maintenance of crude hemolysate at 20 to 25 degrees C in the presence of EDTA and KCl increased NAD synthetase stability substantially ( half-life = 10 days ) .
	manualset3
150385	6	409883	7	NULL	NULL	0	NULL	24 hours 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme was found to be cold labile and extremely unstable in crude hemolysate , with complete loss of activity occurring after 24 hours at 4 degrees C. However , maintenance of crude hemolysate at 20 to 25 degrees C in the presence of EDTA and KCl increased NAD synthetase stability substantially ( half-life = 10 days ) .
	manualset3
150386	7	409883	7	NULL	NULL	0	NULL	4 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme was found to be cold labile and extremely unstable in crude hemolysate , with complete loss of activity occurring after 24 hours at 4 degrees C. However , maintenance of crude hemolysate at 20 to 25 degrees C in the presence of EDTA and KCl increased NAD synthetase stability substantially ( half-life = 10 days ) .
	manualset3
150387	8	409883	7	NULL	NULL	0	NULL	crude hemolysate	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme was found to be cold labile and extremely unstable in crude hemolysate , with complete loss of activity occurring after 24 hours at 4 degrees C. However , maintenance of crude hemolysate at 20 to 25 degrees C in the presence of EDTA and KCl increased NAD synthetase stability substantially ( half-life = 10 days ) .
	manualset3
150388	9	409883	7	NULL	NULL	0	NULL	 20 to 25 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme was found to be cold labile and extremely unstable in crude hemolysate , with complete loss of activity occurring after 24 hours at 4 degrees C. However , maintenance of crude hemolysate at 20 to 25 degrees C in the presence of EDTA and KCl increased NAD synthetase stability substantially ( half-life = 10 days ) .
	manualset3
150389	10	409883	7	NULL	NULL	0	NULL	EDTA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme was found to be cold labile and extremely unstable in crude hemolysate , with complete loss of activity occurring after 24 hours at 4 degrees C. However , maintenance of crude hemolysate at 20 to 25 degrees C in the presence of EDTA and KCl increased NAD synthetase stability substantially ( half-life = 10 days ) .
	manualset3
150390	11	409883	7	NULL	NULL	0	NULL	KCl 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme was found to be cold labile and extremely unstable in crude hemolysate , with complete loss of activity occurring after 24 hours at 4 degrees C. However , maintenance of crude hemolysate at 20 to 25 degrees C in the presence of EDTA and KCl increased NAD synthetase stability substantially ( half-life = 10 days ) .
	manualset3
150391	12	409883	7	NULL	NULL	0	NULL	NAD synthetase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme was found to be cold labile and extremely unstable in crude hemolysate , with complete loss of activity occurring after 24 hours at 4 degrees C. However , maintenance of crude hemolysate at 20 to 25 degrees C in the presence of EDTA and KCl increased NAD synthetase stability substantially ( half-life = 10 days ) .
	manualset3
150392	13	409883	7	NULL	NULL	0	NULL	stability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme was found to be cold labile and extremely unstable in crude hemolysate , with complete loss of activity occurring after 24 hours at 4 degrees C. However , maintenance of crude hemolysate at 20 to 25 degrees C in the presence of EDTA and KCl increased NAD synthetase stability substantially ( half-life = 10 days ) .
	manualset3
150393	1	409884	7	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme was homogeneous by disc gel electrophoresis on polyacrylamide .
	manualset3
150394	2	409884	7	NULL	NULL	0	NULL	disc gel electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme was homogeneous by disc gel electrophoresis on polyacrylamide .
	manualset3
150395	3	409884	7	NULL	NULL	0	NULL	polyacrylamide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme was homogeneous by disc gel electrophoresis on polyacrylamide .
	manualset3
150396	1	409885	7	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme was incubated with ( 10-DR-3H ) - or ( 10-LS-3H ) - labeled arachidonic acid , and 6-trans-LTB4 and its 12-epimer were analyzed .
	manualset3
150397	2	409885	7	NULL	NULL	0	NULL	( 10-DR-3H )  labeled arachidonic acid	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme was incubated with ( 10-DR-3H ) - or ( 10-LS-3H ) - labeled arachidonic acid , and 6-trans-LTB4 and its 12-epimer were analyzed .
	manualset3
150398	3	409885	7	NULL	NULL	0	NULL	( 10-LS-3H ) - labeled arachidonic acid	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme was incubated with ( 10-DR-3H ) - or ( 10-LS-3H ) - labeled arachidonic acid , and 6-trans-LTB4 and its 12-epimer were analyzed .
	manualset3
150399	4	409885	7	NULL	NULL	0	NULL	6-trans-LTB4	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme was incubated with ( 10-DR-3H ) - or ( 10-LS-3H ) - labeled arachidonic acid , and 6-trans-LTB4 and its 12-epimer were analyzed .
	manualset3
150400	5	409885	7	NULL	NULL	0	NULL	12-epimer	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme was incubated with ( 10-DR-3H ) - or ( 10-LS-3H ) - labeled arachidonic acid , and 6-trans-LTB4 and its 12-epimer were analyzed .
	manualset3
150401	6	409885	7	NULL	NULL	0	NULL	analyzed	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme was incubated with ( 10-DR-3H ) - or ( 10-LS-3H ) - labeled arachidonic acid , and 6-trans-LTB4 and its 12-epimer were analyzed .
	manualset3
150402	1	409886	7	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzyme was shown to be inhibited in the presence of EDTA and to have a pH optimum of 7.5 .
	manualset3
150404	2	409886	7	NULL	NULL	NULL	NULL	EDTA	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme was shown to be inhibited in the presence of EDTA and to have a pH optimum of 7.5 .
	manualset3
150405	3	409886	7	NULL	NULL	NULL	NULL	pH optimum of 7.5	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzyme was shown to be inhibited in the presence of EDTA and to have a pH optimum of 7.5 .
	manualset3
150406	1	409887	7	NULL	NULL	0	NULL	enzymes	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzymes downstream of cyclooxygenase-2 may determine the PGE2/PGF2alpha ratio in the porcine uterus .
	manualset3
150408	3	409887	7	NULL	NULL	0	NULL	cyclooxygenase-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzymes downstream of cyclooxygenase-2 may determine the PGE2/PGF2alpha ratio in the porcine uterus .
	manualset3
150409	4	409887	7	NULL	NULL	0	NULL	PGE2/PGF2alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzymes downstream of cyclooxygenase-2 may determine the PGE2/PGF2alpha ratio in the porcine uterus .
	manualset3
150410	5	409887	7	NULL	NULL	NULL	NULL	 porcine uterus	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzymes downstream of cyclooxygenase-2 may determine the PGE2/PGF2alpha ratio in the porcine uterus .
	manualset3
150412	1	409888	7	NULL	NULL	0	NULL	enzymic properties	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzymic properties of the modified protein are similar to those of RNase A. It is shown that the pK of the fluorescein group can be used as an index of protein conformation to monitor structural changes in the protein .
	manualset3
150413	2	409888	7	NULL	NULL	0	NULL	modified protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzymic properties of the modified protein are similar to those of RNase A. It is shown that the pK of the fluorescein group can be used as an index of protein conformation to monitor structural changes in the protein .
	manualset3
150414	3	409888	7	NULL	NULL	0	NULL	RNase A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzymic properties of the modified protein are similar to those of RNase A. It is shown that the pK of the fluorescein group can be used as an index of protein conformation to monitor structural changes in the protein .
	manualset3
150415	4	409888	7	NULL	NULL	NULL	NULL	 pK	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzymic properties of the modified protein are similar to those of RNase A. It is shown that the pK of the fluorescein group can be used as an index of protein conformation to monitor structural changes in the protein .
	manualset3
150416	5	409888	7	NULL	NULL	0	NULL	fluorescein group	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzymic properties of the modified protein are similar to those of RNase A. It is shown that the pK of the fluorescein group can be used as an index of protein conformation to monitor structural changes in the protein .
	manualset3
150417	6	409888	7	NULL	NULL	0	NULL	protein conformation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzymic properties of the modified protein are similar to those of RNase A. It is shown that the pK of the fluorescein group can be used as an index of protein conformation to monitor structural changes in the protein .
	manualset3
150418	7	409888	7	NULL	NULL	NULL	NULL	structural changes	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The enzymic properties of the modified protein are similar to those of RNase A. It is shown that the pK of the fluorescein group can be used as an index of protein conformation to monitor structural changes in the protein .
	manualset3
150419	8	409888	7	NULL	NULL	0	NULL	protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzymic properties of the modified protein are similar to those of RNase A. It is shown that the pK of the fluorescein group can be used as an index of protein conformation to monitor structural changes in the protein .
	manualset3
157157	9	409888	7	NULL	NULL	0	NULL	index	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The enzymic properties of the modified protein are similar to those of RNase A. It is shown that the pK of the fluorescein group can be used as an index of protein conformation to monitor structural changes in the protein .
	manualset3
150420	1	409889	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A study of nutrient digestibility and growth performance of broiler chicks fed hairy and hairless canary seed ( Phalaris canariensis L. ) products .
	manualset3
150421	2	409889	7	NULL	NULL	0	NULL	nutrient digestibility	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A study of nutrient digestibility and growth performance of broiler chicks fed hairy and hairless canary seed ( Phalaris canariensis L. ) products .
	manualset3
150422	3	409889	7	NULL	NULL	0	NULL	growth performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A study of nutrient digestibility and growth performance of broiler chicks fed hairy and hairless canary seed ( Phalaris canariensis L. ) products .
	manualset3
150423	4	409889	7	NULL	NULL	0	NULL	broiler chicks	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A study of nutrient digestibility and growth performance of broiler chicks fed hairy and hairless canary seed ( Phalaris canariensis L. ) products .
	manualset3
150424	5	409889	7	NULL	NULL	NULL	NULL	hairy canary seed products	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A study of nutrient digestibility and growth performance of broiler chicks fed hairy and hairless canary seed ( Phalaris canariensis L. ) products .
	manualset3
150425	6	409889	7	NULL	NULL	NULL	NULL	hairless canary seed products	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A study of nutrient digestibility and growth performance of broiler chicks fed hairy and hairless canary seed ( Phalaris canariensis L. ) products .
	manualset3
150426	7	409889	7	NULL	NULL	0	NULL	Phalaris canariensis L. 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A study of nutrient digestibility and growth performance of broiler chicks fed hairy and hairless canary seed ( Phalaris canariensis L. ) products .
	manualset3
150427	1	409890	7	NULL	NULL	NULL	NULL	epidemiological patterns 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The epidemiological and clinical patterns of HIV infection / AIDS in Korea was investigated by retrospectively analyzing the medical records of 176 HIV-infected persons who visited two major referral hospitals of AIDS in Korea from 1985 to April 2000 .
	manualset3
150428	2	409890	7	NULL	NULL	NULL	NULL	clinical patterns 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The epidemiological and clinical patterns of HIV infection / AIDS in Korea was investigated by retrospectively analyzing the medical records of 176 HIV-infected persons who visited two major referral hospitals of AIDS in Korea from 1985 to April 2000 .
	manualset3
150430	5	409890	7	NULL	NULL	NULL	NULL	Korea	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The epidemiological and clinical patterns of HIV infection / AIDS in Korea was investigated by retrospectively analyzing the medical records of 176 HIV-infected persons who visited two major referral hospitals of AIDS in Korea from 1985 to April 2000 .
	manualset3
150445	6	409890	7	NULL	NULL	NULL	NULL	medical records 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The epidemiological and clinical patterns of HIV infection / AIDS in Korea was investigated by retrospectively analyzing the medical records of 176 HIV-infected persons who visited two major referral hospitals of AIDS in Korea from 1985 to April 2000 .
	manualset3
150447	7	409890	7	NULL	NULL	NULL	NULL	176 HIV-infected persons	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The epidemiological and clinical patterns of HIV infection / AIDS in Korea was investigated by retrospectively analyzing the medical records of 176 HIV-infected persons who visited two major referral hospitals of AIDS in Korea from 1985 to April 2000 .
	manualset3
150456	8	409890	7	NULL	NULL	NULL	NULL	major referral hospitals	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The epidemiological and clinical patterns of HIV infection / AIDS in Korea was investigated by retrospectively analyzing the medical records of 176 HIV-infected persons who visited two major referral hospitals of AIDS in Korea from 1985 to April 2000 .
	manualset3
150458	9	409890	7	NULL	NULL	NULL	NULL	AIDS	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The epidemiological and clinical patterns of HIV infection / AIDS in Korea was investigated by retrospectively analyzing the medical records of 176 HIV-infected persons who visited two major referral hospitals of AIDS in Korea from 1985 to April 2000 .
	manualset3
150462	10	409890	7	NULL	NULL	NULL	NULL	Korea	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The epidemiological and clinical patterns of HIV infection / AIDS in Korea was investigated by retrospectively analyzing the medical records of 176 HIV-infected persons who visited two major referral hospitals of AIDS in Korea from 1985 to April 2000 .
	manualset3
150463	11	409890	7	NULL	NULL	NULL	NULL	1985 to April 2000	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The epidemiological and clinical patterns of HIV infection / AIDS in Korea was investigated by retrospectively analyzing the medical records of 176 HIV-infected persons who visited two major referral hospitals of AIDS in Korea from 1985 to April 2000 .
	manualset3
152233	3	409890	7	NULL	NULL	NULL	NULL	HIV infection / AIDS	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The epidemiological and clinical patterns of HIV infection / AIDS in Korea was investigated by retrospectively analyzing the medical records of 176 HIV-infected persons who visited two major referral hospitals of AIDS in Korea from 1985 to April 2000 .
	manualset3
150467	1	409891	7	NULL	NULL	0	NULL	epidemiology of accidents	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The epidemiology of accidents -- a survey in Aviemore .
	manualset3
150469	2	409891	7	NULL	NULL	NULL	NULL	survey	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The epidemiology of accidents -- a survey in Aviemore .
	manualset3
150472	3	409891	7	NULL	NULL	0	NULL	Aviemore	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The epidemiology of accidents -- a survey in Aviemore .
	manualset3
150620	1	409892	7	NULL	NULL	0	NULL	epidemiology	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The epidemiology of ankle injuries in professional rugby union players .
	manualset3
150621	2	409892	7	NULL	NULL	0	NULL	ankle injuries	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The epidemiology of ankle injuries in professional rugby union players .
	manualset3
150622	3	409892	7	NULL	NULL	0	NULL	professional rugby union players	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The epidemiology of ankle injuries in professional rugby union players .
	manualset3
150623	1	409893	7	NULL	NULL	0	NULL	epidermal dimer action spectra	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The epidermal dimer action spectra were compared with erythema action spectra determined from the same volunteers and ultraviolet radiation sources .
	manualset3
150624	2	409893	7	NULL	NULL	0	NULL	erythema action spectra	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The epidermal dimer action spectra were compared with erythema action spectra determined from the same volunteers and ultraviolet radiation sources .
	manualset3
150625	3	409893	7	NULL	NULL	0	NULL	volunteers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The epidermal dimer action spectra were compared with erythema action spectra determined from the same volunteers and ultraviolet radiation sources .
	manualset3
150626	4	409893	7	NULL	NULL	0	NULL	ultraviolet radiation sources	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The epidermal dimer action spectra were compared with erythema action spectra determined from the same volunteers and ultraviolet radiation sources .
	manualset3
150627	1	409894	7	NULL	NULL	NULL	NULL	epigenome 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The epigenome of cancer cells is determined by DNA methylation and an array of post-translational modifications of the core histones .
	manualset3
150628	3	409894	7	NULL	NULL	NULL	NULL	DNA methylation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The epigenome of cancer cells is determined by DNA methylation and an array of post-translational modifications of the core histones .
	manualset3
150629	4	409894	7	NULL	NULL	NULL	NULL	array	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The epigenome of cancer cells is determined by DNA methylation and an array of post-translational modifications of the core histones .
	manualset3
150630	5	409894	7	NULL	NULL	NULL	NULL	post-translational modifications	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The epigenome of cancer cells is determined by DNA methylation and an array of post-translational modifications of the core histones .
	manualset3
150631	6	409894	7	NULL	NULL	NULL	NULL	core histones	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The epigenome of cancer cells is determined by DNA methylation and an array of post-translational modifications of the core histones .
	manualset3
152235	2	409894	7	NULL	NULL	0	NULL	Cancer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The epigenome of cancer cells is determined by DNA methylation and an array of post-translational modifications of the core histones .
	manualset3
150632	1	409895	7	NULL	NULL	NULL	NULL	equations 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The equations contain three dimensionless numbers determined by the physiology of the epithelium and cortex cells .
	manualset3
150633	2	409895	7	NULL	NULL	0	NULL	three dimensionless numbers 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The equations contain three dimensionless numbers determined by the physiology of the epithelium and cortex cells .
	manualset3
150634	3	409895	7	NULL	NULL	NULL	NULL	physiology of the epithelium cells	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The equations contain three dimensionless numbers determined by the physiology of the epithelium and cortex cells .
	manualset3
150635	4	409895	7	NULL	NULL	NULL	NULL	physiology of the cortex cells	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The equations contain three dimensionless numbers determined by the physiology of the epithelium and cortex cells .
	manualset3
150636	1	409896	7	NULL	NULL	NULL	NULL	equations	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The equations using DXA measurements provide good estimation ( R ( 2 ) & gt ; 0.70 ) of the weight of fat in the carcass and primal cuts .
	manualset3
150637	2	409896	7	NULL	NULL	NULL	NULL	DXA measurements 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The equations using DXA measurements provide good estimation ( R ( 2 ) & gt ; 0.70 ) of the weight of fat in the carcass and primal cuts .
	manualset3
150638	3	409896	7	NULL	NULL	0	NULL	good estimation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The equations using DXA measurements provide good estimation ( R ( 2 ) & gt ; 0.70 ) of the weight of fat in the carcass and primal cuts .
	manualset3
150639	4	409896	7	NULL	NULL	0	NULL	( R ( 2 ) & gt ; 0.70 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The equations using DXA measurements provide good estimation ( R ( 2 ) & gt ; 0.70 ) of the weight of fat in the carcass and primal cuts .
	manualset3
150640	5	409896	7	NULL	NULL	NULL	NULL	 fat	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The equations using DXA measurements provide good estimation ( R ( 2 ) & gt ; 0.70 ) of the weight of fat in the carcass and primal cuts .
	manualset3
150641	6	409896	7	NULL	NULL	NULL	NULL	carcass	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The equations using DXA measurements provide good estimation ( R ( 2 ) & gt ; 0.70 ) of the weight of fat in the carcass and primal cuts .
	manualset3
150642	7	409896	7	NULL	NULL	0	NULL	 primal cuts	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The equations using DXA measurements provide good estimation ( R ( 2 ) & gt ; 0.70 ) of the weight of fat in the carcass and primal cuts .
	manualset3
157158	8	409896	7	NULL	NULL	0	NULL	weight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The equations using DXA measurements provide good estimation ( R ( 2 ) & gt ; 0.70 ) of the weight of fat in the carcass and primal cuts .
	manualset3
150648	1	409897	7	NULL	NULL	0	NULL	equilibrium dissociation constant	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The equilibrium dissociation constant for channel block by ACh was approximately 2-fold lower in alpha Y190F receptors compared with in wildtype receptors , suggesting that there are changes in the pore region of the receptor as a consequence of the mutation .
	manualset3
150654	2	409897	7	NULL	NULL	0	NULL	channel block	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The equilibrium dissociation constant for channel block by ACh was approximately 2-fold lower in alpha Y190F receptors compared with in wildtype receptors , suggesting that there are changes in the pore region of the receptor as a consequence of the mutation .
	manualset3
150655	3	409897	7	NULL	NULL	0	NULL	ACh	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The equilibrium dissociation constant for channel block by ACh was approximately 2-fold lower in alpha Y190F receptors compared with in wildtype receptors , suggesting that there are changes in the pore region of the receptor as a consequence of the mutation .
	manualset3
150657	4	409897	7	NULL	NULL	0	NULL	alpha Y190F receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The equilibrium dissociation constant for channel block by ACh was approximately 2-fold lower in alpha Y190F receptors compared with in wildtype receptors , suggesting that there are changes in the pore region of the receptor as a consequence of the mutation .
	manualset3
150658	5	409897	7	NULL	NULL	0	NULL	wildtype receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The equilibrium dissociation constant for channel block by ACh was approximately 2-fold lower in alpha Y190F receptors compared with in wildtype receptors , suggesting that there are changes in the pore region of the receptor as a consequence of the mutation .
	manualset3
150761	7	409897	7	NULL	NULL	NULL	NULL	 pore region of the receptor	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The equilibrium dissociation constant for channel block by ACh was approximately 2-fold lower in alpha Y190F receptors compared with in wildtype receptors , suggesting that there are changes in the pore region of the receptor as a consequence of the mutation .
	manualset3
150762	9	409897	7	NULL	NULL	NULL	NULL	mutation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The equilibrium dissociation constant for channel block by ACh was approximately 2-fold lower in alpha Y190F receptors compared with in wildtype receptors , suggesting that there are changes in the pore region of the receptor as a consequence of the mutation .
	manualset3
157159	6	409897	7	NULL	NULL	NULL	NULL	changes	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The equilibrium dissociation constant for channel block by ACh was approximately 2-fold lower in alpha Y190F receptors compared with in wildtype receptors , suggesting that there are changes in the pore region of the receptor as a consequence of the mutation .
	manualset3
157160	8	409897	7	NULL	NULL	0	NULL	consequence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The equilibrium dissociation constant for channel block by ACh was approximately 2-fold lower in alpha Y190F receptors compared with in wildtype receptors , suggesting that there are changes in the pore region of the receptor as a consequence of the mutation .
	manualset3
150775	1	409898	7	NULL	NULL	0	NULL	eradication 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The eradication of variola was defined as eradication of clinical forms of smallpox not as the final eradication of the variola virus .
	manualset3
150777	2	409898	7	NULL	NULL	0	NULL	variola	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The eradication of variola was defined as eradication of clinical forms of smallpox not as the final eradication of the variola virus .
	manualset3
150779	3	409898	7	NULL	NULL	0	NULL	eradication 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The eradication of variola was defined as eradication of clinical forms of smallpox not as the final eradication of the variola virus .
	manualset3
150781	4	409898	7	NULL	NULL	0	NULL	clinical forms of smallpox	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The eradication of variola was defined as eradication of clinical forms of smallpox not as the final eradication of the variola virus .
	manualset3
150787	5	409898	7	NULL	NULL	0	NULL	final eradication	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The eradication of variola was defined as eradication of clinical forms of smallpox not as the final eradication of the variola virus .
	manualset3
150789	6	409898	7	NULL	NULL	0	NULL	variola virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The eradication of variola was defined as eradication of clinical forms of smallpox not as the final eradication of the variola virus .
	manualset3
150815	1	409899	7	NULL	NULL	0	NULL	eradication rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The eradication rates were 54.5 % in the monotherapy group , and 81.3 % in the combination therapy group .
	manualset3
150816	2	409899	7	NULL	NULL	0	NULL	54.5 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The eradication rates were 54.5 % in the monotherapy group , and 81.3 % in the combination therapy group .
	manualset3
150817	3	409899	7	NULL	NULL	0	NULL	monotherapy group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The eradication rates were 54.5 % in the monotherapy group , and 81.3 % in the combination therapy group .
	manualset3
150818	4	409899	7	NULL	NULL	0	NULL	81.3 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The eradication rates were 54.5 % in the monotherapy group , and 81.3 % in the combination therapy group .
	manualset3
150819	5	409899	7	NULL	NULL	0	NULL	combination therapy group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The eradication rates were 54.5 % in the monotherapy group , and 81.3 % in the combination therapy group .
	manualset3
150820	1	409900	7	NULL	NULL	0	NULL	erythrocyte membranes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The erythrocyte membranes showed a high cholesterol/phospholipid ratio , with no significant susceptibility to lipid peroxidation in vitro .
	manualset3
150821	2	409900	7	NULL	NULL	0	NULL	high cholesterol/phospholipid ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The erythrocyte membranes showed a high cholesterol/phospholipid ratio , with no significant susceptibility to lipid peroxidation in vitro .
	manualset3
150822	4	409900	7	NULL	NULL	NULL	NULL	lipid peroxidation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The erythrocyte membranes showed a high cholesterol/phospholipid ratio , with no significant susceptibility to lipid peroxidation in vitro .
	manualset3
150824	3	409900	7	NULL	NULL	NULL	NULL	significant susceptibility	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The erythrocyte membranes showed a high cholesterol/phospholipid ratio , with no significant susceptibility to lipid peroxidation in vitro .
	manualset3
150843	1	409901	7	NULL	NULL	NULL	NULL	escape probability	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The escape probability out of the superconducting state of a hysteretic dc SQUID has been measured at different values of the applied magnetic flux .
	manualset3
150844	2	409901	7	NULL	NULL	0	NULL	superconducting state	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The escape probability out of the superconducting state of a hysteretic dc SQUID has been measured at different values of the applied magnetic flux .
	manualset3
150845	3	409901	7	NULL	NULL	0	NULL	hysteretic dc SQUID	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The escape probability out of the superconducting state of a hysteretic dc SQUID has been measured at different values of the applied magnetic flux .
	manualset3
150846	4	409901	7	NULL	NULL	NULL	NULL	different values	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The escape probability out of the superconducting state of a hysteretic dc SQUID has been measured at different values of the applied magnetic flux .
	manualset3
150847	5	409901	7	NULL	NULL	0	NULL	applied magnetic flux	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The escape probability out of the superconducting state of a hysteretic dc SQUID has been measured at different values of the applied magnetic flux .
	manualset3
150848	1	409902	7	NULL	NULL	0	NULL	essential role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The essential role of hydrodynamic shear force in the formation of biofilm and granular sludge .
	manualset3
150849	2	409902	7	NULL	NULL	0	NULL	hydrodynamic shear force	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The essential role of hydrodynamic shear force in the formation of biofilm and granular sludge .
	manualset3
150850	3	409902	7	NULL	NULL	0	NULL	formation of biofilm	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The essential role of hydrodynamic shear force in the formation of biofilm and granular sludge .
	manualset3
150851	4	409902	7	NULL	NULL	0	NULL	granular sludge	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The essential role of hydrodynamic shear force in the formation of biofilm and granular sludge .
	manualset3
150852	1	409903	7	NULL	NULL	NULL	NULL	establishment 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The establishment of a cardiac prognosis that is significantly worse than that following heart transplant is central in the determination of candidacy for transplantation .
	manualset3
150853	2	409903	7	NULL	NULL	0	NULL	cardiac prognosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The establishment of a cardiac prognosis that is significantly worse than that following heart transplant is central in the determination of candidacy for transplantation .
	manualset3
150854	3	409903	7	NULL	NULL	0	NULL	heart transplant	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The establishment of a cardiac prognosis that is significantly worse than that following heart transplant is central in the determination of candidacy for transplantation .
	manualset3
150855	4	409903	7	NULL	NULL	NULL	NULL	determination of candidacy	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The establishment of a cardiac prognosis that is significantly worse than that following heart transplant is central in the determination of candidacy for transplantation .
	manualset3
150856	5	409903	7	NULL	NULL	0	NULL	transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The establishment of a cardiac prognosis that is significantly worse than that following heart transplant is central in the determination of candidacy for transplantation .
	manualset3
150857	1	409904	7	NULL	NULL	0	NULL	 study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A study of tetany should include the protein metabolism as well as that of the inorganic salts , since it seems possible that the tetany is due to protein split-products and not to the alkalosis .
	manualset3
150858	2	409904	7	NULL	NULL	0	NULL	tetany	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A study of tetany should include the protein metabolism as well as that of the inorganic salts , since it seems possible that the tetany is due to protein split-products and not to the alkalosis .
	manualset3
150859	3	409904	7	NULL	NULL	0	NULL	protein metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A study of tetany should include the protein metabolism as well as that of the inorganic salts , since it seems possible that the tetany is due to protein split-products and not to the alkalosis .
	manualset3
150860	4	409904	7	NULL	NULL	0	NULL	inorganic salts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A study of tetany should include the protein metabolism as well as that of the inorganic salts , since it seems possible that the tetany is due to protein split-products and not to the alkalosis .
	manualset3
150861	5	409904	7	NULL	NULL	0	NULL	tetany	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A study of tetany should include the protein metabolism as well as that of the inorganic salts , since it seems possible that the tetany is due to protein split-products and not to the alkalosis .
	manualset3
150862	6	409904	7	NULL	NULL	0	NULL	protein split-products	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A study of tetany should include the protein metabolism as well as that of the inorganic salts , since it seems possible that the tetany is due to protein split-products and not to the alkalosis .
	manualset3
150863	7	409904	7	NULL	NULL	0	NULL	alkalosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A study of tetany should include the protein metabolism as well as that of the inorganic salts , since it seems possible that the tetany is due to protein split-products and not to the alkalosis .
	manualset3
150864	1	409905	7	NULL	NULL	0	NULL	establishment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The establishment of a threshold voltage enabled the differentiation of two similar cationic species : Methyl Green and Neutral Red .
	manualset3
150865	2	409905	7	NULL	NULL	0	NULL	threshold voltage	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The establishment of a threshold voltage enabled the differentiation of two similar cationic species : Methyl Green and Neutral Red .
	manualset3
150866	3	409905	7	NULL	NULL	0	NULL	differentiation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The establishment of a threshold voltage enabled the differentiation of two similar cationic species : Methyl Green and Neutral Red .
	manualset3
150867	4	409905	7	NULL	NULL	0	NULL	two similar cationic species	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The establishment of a threshold voltage enabled the differentiation of two similar cationic species : Methyl Green and Neutral Red .
	manualset3
150868	5	409905	7	NULL	NULL	0	NULL	Methyl Green	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The establishment of a threshold voltage enabled the differentiation of two similar cationic species : Methyl Green and Neutral Red .
	manualset3
150869	6	409905	7	NULL	NULL	0	NULL	Neutral Red	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The establishment of a threshold voltage enabled the differentiation of two similar cationic species : Methyl Green and Neutral Red .
	manualset3
150976	1	409906	7	NULL	NULL	NULL	NULL	estimated incremental costs	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The estimated incremental costs per death avoided were as follows : single-donor apheresis platelets , $ 15 million ; solvent detergent plasma , $ 17 million ; leukocyte-reduced transfusions in cardiac surgery , $ 11 , 000 ; HIV-1 antibody testing , $ 22 , 000 ; and HIV-1 antigen testing , $ 3.9 million .
	manualset3
150982	2	409906	7	NULL	NULL	0	NULL	death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The estimated incremental costs per death avoided were as follows : single-donor apheresis platelets , $ 15 million ; solvent detergent plasma , $ 17 million ; leukocyte-reduced transfusions in cardiac surgery , $ 11 , 000 ; HIV-1 antibody testing , $ 22 , 000 ; and HIV-1 antigen testing , $ 3.9 million .
	manualset3
150983	3	409906	7	NULL	NULL	0	NULL	single-donor apheresis platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The estimated incremental costs per death avoided were as follows : single-donor apheresis platelets , $ 15 million ; solvent detergent plasma , $ 17 million ; leukocyte-reduced transfusions in cardiac surgery , $ 11 , 000 ; HIV-1 antibody testing , $ 22 , 000 ; and HIV-1 antigen testing , $ 3.9 million .
	manualset3
150984	4	409906	7	NULL	NULL	0	NULL	$ 15 million	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The estimated incremental costs per death avoided were as follows : single-donor apheresis platelets , $ 15 million ; solvent detergent plasma , $ 17 million ; leukocyte-reduced transfusions in cardiac surgery , $ 11 , 000 ; HIV-1 antibody testing , $ 22 , 000 ; and HIV-1 antigen testing , $ 3.9 million .
	manualset3
150985	5	409906	7	NULL	NULL	NULL	NULL	solvent detergent plasma	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The estimated incremental costs per death avoided were as follows : single-donor apheresis platelets , $ 15 million ; solvent detergent plasma , $ 17 million ; leukocyte-reduced transfusions in cardiac surgery , $ 11 , 000 ; HIV-1 antibody testing , $ 22 , 000 ; and HIV-1 antigen testing , $ 3.9 million .
	manualset3
151024	6	409906	7	NULL	NULL	0	NULL	 $ 17 million	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The estimated incremental costs per death avoided were as follows : single-donor apheresis platelets , $ 15 million ; solvent detergent plasma , $ 17 million ; leukocyte-reduced transfusions in cardiac surgery , $ 11 , 000 ; HIV-1 antibody testing , $ 22 , 000 ; and HIV-1 antigen testing , $ 3.9 million .
	manualset3
151025	7	409906	7	NULL	NULL	0	NULL	leukocyte-reduced transfusions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The estimated incremental costs per death avoided were as follows : single-donor apheresis platelets , $ 15 million ; solvent detergent plasma , $ 17 million ; leukocyte-reduced transfusions in cardiac surgery , $ 11 , 000 ; HIV-1 antibody testing , $ 22 , 000 ; and HIV-1 antigen testing , $ 3.9 million .
	manualset3
151026	8	409906	7	NULL	NULL	0	NULL	cardiac surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The estimated incremental costs per death avoided were as follows : single-donor apheresis platelets , $ 15 million ; solvent detergent plasma , $ 17 million ; leukocyte-reduced transfusions in cardiac surgery , $ 11 , 000 ; HIV-1 antibody testing , $ 22 , 000 ; and HIV-1 antigen testing , $ 3.9 million .
	manualset3
151029	9	409906	7	NULL	NULL	0	NULL	$ 11 , 000	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The estimated incremental costs per death avoided were as follows : single-donor apheresis platelets , $ 15 million ; solvent detergent plasma , $ 17 million ; leukocyte-reduced transfusions in cardiac surgery , $ 11 , 000 ; HIV-1 antibody testing , $ 22 , 000 ; and HIV-1 antigen testing , $ 3.9 million .
	manualset3
151030	10	409906	7	NULL	NULL	0	NULL	HIV-1 antibody testing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The estimated incremental costs per death avoided were as follows : single-donor apheresis platelets , $ 15 million ; solvent detergent plasma , $ 17 million ; leukocyte-reduced transfusions in cardiac surgery , $ 11 , 000 ; HIV-1 antibody testing , $ 22 , 000 ; and HIV-1 antigen testing , $ 3.9 million .
	manualset3
151032	11	409906	7	NULL	NULL	0	NULL	$ 22 , 000 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The estimated incremental costs per death avoided were as follows : single-donor apheresis platelets , $ 15 million ; solvent detergent plasma , $ 17 million ; leukocyte-reduced transfusions in cardiac surgery , $ 11 , 000 ; HIV-1 antibody testing , $ 22 , 000 ; and HIV-1 antigen testing , $ 3.9 million .
	manualset3
151036	12	409906	7	NULL	NULL	NULL	NULL	HIV-1 antigen testing	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The estimated incremental costs per death avoided were as follows : single-donor apheresis platelets , $ 15 million ; solvent detergent plasma , $ 17 million ; leukocyte-reduced transfusions in cardiac surgery , $ 11 , 000 ; HIV-1 antibody testing , $ 22 , 000 ; and HIV-1 antigen testing , $ 3.9 million .
	manualset3
151037	13	409906	7	NULL	NULL	0	NULL	$ 3.9 million	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The estimated incremental costs per death avoided were as follows : single-donor apheresis platelets , $ 15 million ; solvent detergent plasma , $ 17 million ; leukocyte-reduced transfusions in cardiac surgery , $ 11 , 000 ; HIV-1 antibody testing , $ 22 , 000 ; and HIV-1 antigen testing , $ 3.9 million .
	manualset3
151040	1	409907	7	NULL	NULL	0	NULL	estimated purification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The estimated purification was about 80 , 000 fold and consistent with the expected Bmax for a pure Mr = 80 , 000 protein binding one CCK molecule .
	manualset3
151041	2	409907	7	NULL	NULL	0	NULL	80 , 000 fold	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The estimated purification was about 80 , 000 fold and consistent with the expected Bmax for a pure Mr = 80 , 000 protein binding one CCK molecule .
	manualset3
151045	3	409907	7	NULL	NULL	0	NULL	expected Bmax	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The estimated purification was about 80 , 000 fold and consistent with the expected Bmax for a pure Mr = 80 , 000 protein binding one CCK molecule .
	manualset3
151050	4	409907	7	NULL	NULL	NULL	NULL	pure 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The estimated purification was about 80 , 000 fold and consistent with the expected Bmax for a pure Mr = 80 , 000 protein binding one CCK molecule .
	manualset3
151051	5	409907	7	NULL	NULL	NULL	NULL	Mr = 80 , 000 protein binding	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The estimated purification was about 80 , 000 fold and consistent with the expected Bmax for a pure Mr = 80 , 000 protein binding one CCK molecule .
	manualset3
151053	6	409907	7	NULL	NULL	NULL	NULL	one CCK molecule	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The estimated purification was about 80 , 000 fold and consistent with the expected Bmax for a pure Mr = 80 , 000 protein binding one CCK molecule .
	manualset3
151054	1	409908	7	NULL	NULL	0	NULL	estimated requirements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The estimated requirements were different ( P & lt ; .05 ) between sexes : .69 % for barrows and .75 % for gilts .
	manualset3
151055	2	409908	7	NULL	NULL	0	NULL	( P & lt ; .05 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The estimated requirements were different ( P & lt ; .05 ) between sexes : .69 % for barrows and .75 % for gilts .
	manualset3
151056	3	409908	7	NULL	NULL	NULL	NULL	sexes 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The estimated requirements were different ( P & lt ; .05 ) between sexes : .69 % for barrows and .75 % for gilts .
	manualset3
151057	5	409908	7	NULL	NULL	NULL	NULL	barrows	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The estimated requirements were different ( P & lt ; .05 ) between sexes : .69 % for barrows and .75 % for gilts .
	manualset3
151058	4	409908	7	NULL	NULL	0	NULL	.69 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The estimated requirements were different ( P & lt ; .05 ) between sexes : .69 % for barrows and .75 % for gilts .
	manualset3
151059	6	409908	7	NULL	NULL	0	NULL	.75 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The estimated requirements were different ( P & lt ; .05 ) between sexes : .69 % for barrows and .75 % for gilts .
	manualset3
151060	7	409908	7	NULL	NULL	0	NULL	gilts	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The estimated requirements were different ( P & lt ; .05 ) between sexes : .69 % for barrows and .75 % for gilts .
	manualset3
151061	1	409909	7	NULL	NULL	0	NULL	estimation procedure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The estimation procedure entailed identifying work areas within each manufacturing process , historical changes in exposure potential and specific tasks involving exposure , and using mathematical models to calculate job - and time-period-specific average exposures .
	manualset3
151062	2	409909	7	NULL	NULL	NULL	NULL	work areas 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The estimation procedure entailed identifying work areas within each manufacturing process , historical changes in exposure potential and specific tasks involving exposure , and using mathematical models to calculate job - and time-period-specific average exposures .
	manualset3
151063	3	409909	7	NULL	NULL	0	NULL	manufacturing process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The estimation procedure entailed identifying work areas within each manufacturing process , historical changes in exposure potential and specific tasks involving exposure , and using mathematical models to calculate job - and time-period-specific average exposures .
	manualset3
151064	4	409909	7	NULL	NULL	0	NULL	historical changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The estimation procedure entailed identifying work areas within each manufacturing process , historical changes in exposure potential and specific tasks involving exposure , and using mathematical models to calculate job - and time-period-specific average exposures .
	manualset3
151065	5	409909	7	NULL	NULL	NULL	NULL	exposure potential 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The estimation procedure entailed identifying work areas within each manufacturing process , historical changes in exposure potential and specific tasks involving exposure , and using mathematical models to calculate job - and time-period-specific average exposures .
	manualset3
151069	6	409909	7	NULL	NULL	0	NULL	specific tasks	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The estimation procedure entailed identifying work areas within each manufacturing process , historical changes in exposure potential and specific tasks involving exposure , and using mathematical models to calculate job - and time-period-specific average exposures .
	manualset3
151076	7	409909	7	NULL	NULL	NULL	NULL	exposure	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The estimation procedure entailed identifying work areas within each manufacturing process , historical changes in exposure potential and specific tasks involving exposure , and using mathematical models to calculate job - and time-period-specific average exposures .
	manualset3
151077	8	409909	7	NULL	NULL	0	NULL	mathematical models	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The estimation procedure entailed identifying work areas within each manufacturing process , historical changes in exposure potential and specific tasks involving exposure , and using mathematical models to calculate job - and time-period-specific average exposures .
	manualset3
151078	9	409909	7	NULL	NULL	NULL	NULL	job - specific average exposures	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The estimation procedure entailed identifying work areas within each manufacturing process , historical changes in exposure potential and specific tasks involving exposure , and using mathematical models to calculate job - and time-period-specific average exposures .
	manualset3
151080	10	409909	7	NULL	NULL	NULL	NULL	time-period-specific average exposures	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The estimation procedure entailed identifying work areas within each manufacturing process , historical changes in exposure potential and specific tasks involving exposure , and using mathematical models to calculate job - and time-period-specific average exposures .
	manualset3
151108	1	409910	7	NULL	NULL	0	NULL	 estrogen primed tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The estrogen primed tissue , changing from proestrous to oestrous , under known increasing progesterone level and preovulatory LH surge , may led to a sort of balancing action on the varying levels of glycogen synthetase and phosphorylase enzyme activities so as to play a role in maintaining a steady state of glycogen concentration in the salivary gland .
	manualset3
151113	2	409910	7	NULL	NULL	0	NULL	proestrous	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The estrogen primed tissue , changing from proestrous to oestrous , under known increasing progesterone level and preovulatory LH surge , may led to a sort of balancing action on the varying levels of glycogen synthetase and phosphorylase enzyme activities so as to play a role in maintaining a steady state of glycogen concentration in the salivary gland .
	manualset3
151115	3	409910	7	NULL	NULL	0	NULL	oestrous	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The estrogen primed tissue , changing from proestrous to oestrous , under known increasing progesterone level and preovulatory LH surge , may led to a sort of balancing action on the varying levels of glycogen synthetase and phosphorylase enzyme activities so as to play a role in maintaining a steady state of glycogen concentration in the salivary gland .
	manualset3
151118	4	409910	7	NULL	NULL	NULL	NULL	increasing progesterone level	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The estrogen primed tissue , changing from proestrous to oestrous , under known increasing progesterone level and preovulatory LH surge , may led to a sort of balancing action on the varying levels of glycogen synthetase and phosphorylase enzyme activities so as to play a role in maintaining a steady state of glycogen concentration in the salivary gland .
	manualset3
151121	5	409910	7	NULL	NULL	NULL	NULL	preovulatory LH surge	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The estrogen primed tissue , changing from proestrous to oestrous , under known increasing progesterone level and preovulatory LH surge , may led to a sort of balancing action on the varying levels of glycogen synthetase and phosphorylase enzyme activities so as to play a role in maintaining a steady state of glycogen concentration in the salivary gland .
	manualset3
151125	6	409910	7	NULL	NULL	NULL	NULL	varying levels of glycogen synthetase	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The estrogen primed tissue , changing from proestrous to oestrous , under known increasing progesterone level and preovulatory LH surge , may led to a sort of balancing action on the varying levels of glycogen synthetase and phosphorylase enzyme activities so as to play a role in maintaining a steady state of glycogen concentration in the salivary gland .
	manualset3
151127	7	409910	7	NULL	NULL	NULL	NULL	varying levels of phosphorylase enzyme activities	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The estrogen primed tissue , changing from proestrous to oestrous , under known increasing progesterone level and preovulatory LH surge , may led to a sort of balancing action on the varying levels of glycogen synthetase and phosphorylase enzyme activities so as to play a role in maintaining a steady state of glycogen concentration in the salivary gland .
	manualset3
151128	8	409910	7	NULL	NULL	0	NULL	steady state	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The estrogen primed tissue , changing from proestrous to oestrous , under known increasing progesterone level and preovulatory LH surge , may led to a sort of balancing action on the varying levels of glycogen synthetase and phosphorylase enzyme activities so as to play a role in maintaining a steady state of glycogen concentration in the salivary gland .
	manualset3
151129	9	409910	7	NULL	NULL	0	NULL	glycogen concentration	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The estrogen primed tissue , changing from proestrous to oestrous , under known increasing progesterone level and preovulatory LH surge , may led to a sort of balancing action on the varying levels of glycogen synthetase and phosphorylase enzyme activities so as to play a role in maintaining a steady state of glycogen concentration in the salivary gland .
	manualset3
151130	10	409910	7	NULL	NULL	0	NULL	salivary gland	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The estrogen primed tissue , changing from proestrous to oestrous , under known increasing progesterone level and preovulatory LH surge , may led to a sort of balancing action on the varying levels of glycogen synthetase and phosphorylase enzyme activities so as to play a role in maintaining a steady state of glycogen concentration in the salivary gland .
	manualset3
157161	11	409910	7	NULL	NULL	0	NULL	balancing action	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The estrogen primed tissue , changing from proestrous to oestrous , under known increasing progesterone level and preovulatory LH surge , may led to a sort of balancing action on the varying levels of glycogen synthetase and phosphorylase enzyme activities so as to play a role in maintaining a steady state of glycogen concentration in the salivary gland .
	manualset3
151131	1	409911	7	NULL	NULL	0	NULL	ethicist	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The ethicist facilitates the learning process by using various conversation methods in order to find answers to the case and to develop moral competencies .
	manualset3
151132	2	409911	7	NULL	NULL	NULL	NULL	 learning process	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ethicist facilitates the learning process by using various conversation methods in order to find answers to the case and to develop moral competencies .
	manualset3
151133	3	409911	7	NULL	NULL	NULL	NULL	various conversation methods	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ethicist facilitates the learning process by using various conversation methods in order to find answers to the case and to develop moral competencies .
	manualset3
151134	4	409911	7	NULL	NULL	NULL	NULL	answers	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ethicist facilitates the learning process by using various conversation methods in order to find answers to the case and to develop moral competencies .
	manualset3
151135	5	409911	7	NULL	NULL	0	NULL	case	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The ethicist facilitates the learning process by using various conversation methods in order to find answers to the case and to develop moral competencies .
	manualset3
151136	6	409911	7	NULL	NULL	0	NULL	moral competencies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ethicist facilitates the learning process by using various conversation methods in order to find answers to the case and to develop moral competencies .
	manualset3
151137	1	409912	7	NULL	NULL	0	NULL	ethics	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ethics of off-label use of drugs : oncology pharmacy in Italy .
	manualset3
151138	2	409912	7	NULL	NULL	NULL	NULL	 off-label use	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ethics of off-label use of drugs : oncology pharmacy in Italy .
	manualset3
151139	3	409912	7	NULL	NULL	0	NULL	drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The ethics of off-label use of drugs : oncology pharmacy in Italy .
	manualset3
151140	4	409912	7	NULL	NULL	0	NULL	oncology pharmacy	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The ethics of off-label use of drugs : oncology pharmacy in Italy .
	manualset3
151141	5	409912	7	NULL	NULL	0	NULL	Italy	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The ethics of off-label use of drugs : oncology pharmacy in Italy .
	manualset3
151224	1	409913	7	NULL	NULL	0	NULL	ethylene sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ethylene sensitivity of two WT and the mutants is decreased in the following order : eto1 = WT & lt ; ein3-1 & lt ; ein2-1 = etr1-1 .
	manualset3
151225	2	409913	7	NULL	NULL	0	NULL	two WT	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The ethylene sensitivity of two WT and the mutants is decreased in the following order : eto1 = WT & lt ; ein3-1 & lt ; ein2-1 = etr1-1 .
	manualset3
151226	3	409913	7	NULL	NULL	0	NULL	mutants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The ethylene sensitivity of two WT and the mutants is decreased in the following order : eto1 = WT & lt ; ein3-1 & lt ; ein2-1 = etr1-1 .
	manualset3
151227	4	409913	7	NULL	NULL	0	NULL	following order	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ethylene sensitivity of two WT and the mutants is decreased in the following order : eto1 = WT & lt ; ein3-1 & lt ; ein2-1 = etr1-1 .
	manualset3
151228	5	409913	7	NULL	NULL	0	NULL	eto1 = WT & lt	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ethylene sensitivity of two WT and the mutants is decreased in the following order : eto1 = WT & lt ; ein3-1 & lt ; ein2-1 = etr1-1 .
	manualset3
151229	6	409913	7	NULL	NULL	0	NULL	ein3-1 & lt	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ethylene sensitivity of two WT and the mutants is decreased in the following order : eto1 = WT & lt ; ein3-1 & lt ; ein2-1 = etr1-1 .
	manualset3
151230	7	409913	7	NULL	NULL	0	NULL	ein2-1 = etr1-1	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ethylene sensitivity of two WT and the mutants is decreased in the following order : eto1 = WT & lt ; ein3-1 & lt ; ein2-1 = etr1-1 .
	manualset3
151231	1	409914	7	NULL	NULL	0	NULL	etiology	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The etiology is unclear and there is limited information based on case reports and small case series .
	manualset3
151233	2	409914	7	NULL	NULL	NULL	NULL	information	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The etiology is unclear and there is limited information based on case reports and small case series .
	manualset3
151234	3	409914	7	NULL	NULL	NULL	NULL	case reports	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The etiology is unclear and there is limited information based on case reports and small case series .
	manualset3
151235	4	409914	7	NULL	NULL	NULL	NULL	small case series	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The etiology is unclear and there is limited information based on case reports and small case series .
	manualset3
151236	1	409915	7	NULL	NULL	0	NULL	etiology	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The etiology of this derangement in insulin signaling is related to a chronic inflammatory state , leading to the induction of inducible nitric oxide synthase and release of high levels of nitric oxide and reactive nitrogen species , which together cause posttranslational modifications in the signaling proteins .
	manualset3
151237	2	409915	7	NULL	NULL	0	NULL	derangement in insulin signaling	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The etiology of this derangement in insulin signaling is related to a chronic inflammatory state , leading to the induction of inducible nitric oxide synthase and release of high levels of nitric oxide and reactive nitrogen species , which together cause posttranslational modifications in the signaling proteins .
	manualset3
151238	3	409915	7	NULL	NULL	NULL	NULL	chronic inflammatory state	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The etiology of this derangement in insulin signaling is related to a chronic inflammatory state , leading to the induction of inducible nitric oxide synthase and release of high levels of nitric oxide and reactive nitrogen species , which together cause posttranslational modifications in the signaling proteins .
	manualset3
151239	5	409915	7	NULL	NULL	NULL	NULL	inducible nitric oxide synthase	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The etiology of this derangement in insulin signaling is related to a chronic inflammatory state , leading to the induction of inducible nitric oxide synthase and release of high levels of nitric oxide and reactive nitrogen species , which together cause posttranslational modifications in the signaling proteins .
	manualset3
151240	4	409915	7	NULL	NULL	0	NULL	induction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The etiology of this derangement in insulin signaling is related to a chronic inflammatory state , leading to the induction of inducible nitric oxide synthase and release of high levels of nitric oxide and reactive nitrogen species , which together cause posttranslational modifications in the signaling proteins .
	manualset3
151241	6	409915	7	NULL	NULL	0	NULL	high levels of nitric oxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The etiology of this derangement in insulin signaling is related to a chronic inflammatory state , leading to the induction of inducible nitric oxide synthase and release of high levels of nitric oxide and reactive nitrogen species , which together cause posttranslational modifications in the signaling proteins .
	manualset3
151242	7	409915	7	NULL	NULL	0	NULL	reactive nitrogen species	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The etiology of this derangement in insulin signaling is related to a chronic inflammatory state , leading to the induction of inducible nitric oxide synthase and release of high levels of nitric oxide and reactive nitrogen species , which together cause posttranslational modifications in the signaling proteins .
	manualset3
151243	8	409915	7	NULL	NULL	0	NULL	posttranslational modifications	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The etiology of this derangement in insulin signaling is related to a chronic inflammatory state , leading to the induction of inducible nitric oxide synthase and release of high levels of nitric oxide and reactive nitrogen species , which together cause posttranslational modifications in the signaling proteins .
	manualset3
151244	9	409915	7	NULL	NULL	0	NULL	signaling proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The etiology of this derangement in insulin signaling is related to a chronic inflammatory state , leading to the induction of inducible nitric oxide synthase and release of high levels of nitric oxide and reactive nitrogen species , which together cause posttranslational modifications in the signaling proteins .
	manualset3
151248	1	409916	7	NULL	NULL	0	NULL	evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation and management of the patient with multiple pulmonary nodules are usually guided by the history , physical examination , and laboratory findings .
	manualset3
151250	2	409916	7	NULL	NULL	0	NULL	management	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation and management of the patient with multiple pulmonary nodules are usually guided by the history , physical examination , and laboratory findings .
	manualset3
151252	3	409916	7	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation and management of the patient with multiple pulmonary nodules are usually guided by the history , physical examination , and laboratory findings .
	manualset3
151255	4	409916	7	NULL	NULL	0	NULL	multiple pulmonary nodules	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation and management of the patient with multiple pulmonary nodules are usually guided by the history , physical examination , and laboratory findings .
	manualset3
151256	5	409916	7	NULL	NULL	NULL	NULL	history	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evaluation and management of the patient with multiple pulmonary nodules are usually guided by the history , physical examination , and laboratory findings .
	manualset3
151257	6	409916	7	NULL	NULL	0	NULL	physical examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation and management of the patient with multiple pulmonary nodules are usually guided by the history , physical examination , and laboratory findings .
	manualset3
151258	7	409916	7	NULL	NULL	NULL	NULL	laboratory findings	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evaluation and management of the patient with multiple pulmonary nodules are usually guided by the history , physical examination , and laboratory findings .
	manualset3
151259	1	409917	7	NULL	NULL	0	NULL	evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of CD99 immunoreactivity and EWS/FLI1 translocation by fluorescence in situ hybridization in central PNETs and Ewing 's sarcoma family of tumors .
	manualset3
151260	2	409917	7	NULL	NULL	0	NULL	CD99 immunoreactivity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of CD99 immunoreactivity and EWS/FLI1 translocation by fluorescence in situ hybridization in central PNETs and Ewing 's sarcoma family of tumors .
	manualset3
151261	3	409917	7	NULL	NULL	0	NULL	EWS/FLI1 translocation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of CD99 immunoreactivity and EWS/FLI1 translocation by fluorescence in situ hybridization in central PNETs and Ewing 's sarcoma family of tumors .
	manualset3
151262	4	409917	7	NULL	NULL	NULL	NULL	fluorescence in situ hybridization	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evaluation of CD99 immunoreactivity and EWS/FLI1 translocation by fluorescence in situ hybridization in central PNETs and Ewing 's sarcoma family of tumors .
	manualset3
151263	5	409917	7	NULL	NULL	0	NULL	central PNETs	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of CD99 immunoreactivity and EWS/FLI1 translocation by fluorescence in situ hybridization in central PNETs and Ewing 's sarcoma family of tumors .
	manualset3
151264	6	409917	7	NULL	NULL	0	NULL	Ewing 's sarcoma family of tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of CD99 immunoreactivity and EWS/FLI1 translocation by fluorescence in situ hybridization in central PNETs and Ewing 's sarcoma family of tumors .
	manualset3
151265	1	409918	7	NULL	NULL	0	NULL	evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of Healthy Families Arizona : a multisite home visitation program .
	manualset3
151266	2	409918	7	NULL	NULL	NULL	NULL	Healthy Families 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evaluation of Healthy Families Arizona : a multisite home visitation program .
	manualset3
151267	3	409918	7	NULL	NULL	0	NULL	Arizona	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of Healthy Families Arizona : a multisite home visitation program .
	manualset3
151268	4	409918	7	NULL	NULL	0	NULL	multisite home visitation program	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of Healthy Families Arizona : a multisite home visitation program .
	manualset3
151269	1	409919	7	NULL	NULL	0	NULL	evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of an electron-transfer mediator useful for glucose oxidation is discussed from thermodynamic and kinetic points of view , i.e. the redox potentials of various metal complexes and the second-order rate constants for the electron transfer between GOx in reduced form and the metal complexes in oxidized form .
	manualset3
151270	2	409919	7	NULL	NULL	0	NULL	electron-transfer mediator	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of an electron-transfer mediator useful for glucose oxidation is discussed from thermodynamic and kinetic points of view , i.e. the redox potentials of various metal complexes and the second-order rate constants for the electron transfer between GOx in reduced form and the metal complexes in oxidized form .
	manualset3
151271	3	409919	7	NULL	NULL	0	NULL	 glucose oxidation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of an electron-transfer mediator useful for glucose oxidation is discussed from thermodynamic and kinetic points of view , i.e. the redox potentials of various metal complexes and the second-order rate constants for the electron transfer between GOx in reduced form and the metal complexes in oxidized form .
	manualset3
151277	4	409919	7	NULL	NULL	NULL	NULL	thermodynamic point of view	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evaluation of an electron-transfer mediator useful for glucose oxidation is discussed from thermodynamic and kinetic points of view , i.e. the redox potentials of various metal complexes and the second-order rate constants for the electron transfer between GOx in reduced form and the metal complexes in oxidized form .
	manualset3
151278	5	409919	7	NULL	NULL	NULL	NULL	kinetic points of view	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evaluation of an electron-transfer mediator useful for glucose oxidation is discussed from thermodynamic and kinetic points of view , i.e. the redox potentials of various metal complexes and the second-order rate constants for the electron transfer between GOx in reduced form and the metal complexes in oxidized form .
	manualset3
151286	6	409919	7	NULL	NULL	0	NULL	redox potentials	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of an electron-transfer mediator useful for glucose oxidation is discussed from thermodynamic and kinetic points of view , i.e. the redox potentials of various metal complexes and the second-order rate constants for the electron transfer between GOx in reduced form and the metal complexes in oxidized form .
	manualset3
151287	7	409919	7	NULL	NULL	0	NULL	various metal complexes 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of an electron-transfer mediator useful for glucose oxidation is discussed from thermodynamic and kinetic points of view , i.e. the redox potentials of various metal complexes and the second-order rate constants for the electron transfer between GOx in reduced form and the metal complexes in oxidized form .
	manualset3
151291	8	409919	7	NULL	NULL	NULL	NULL	second-order rate constants	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evaluation of an electron-transfer mediator useful for glucose oxidation is discussed from thermodynamic and kinetic points of view , i.e. the redox potentials of various metal complexes and the second-order rate constants for the electron transfer between GOx in reduced form and the metal complexes in oxidized form .
	manualset3
151294	9	409919	7	NULL	NULL	0	NULL	electron transfer	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of an electron-transfer mediator useful for glucose oxidation is discussed from thermodynamic and kinetic points of view , i.e. the redox potentials of various metal complexes and the second-order rate constants for the electron transfer between GOx in reduced form and the metal complexes in oxidized form .
	manualset3
151296	10	409919	7	NULL	NULL	NULL	NULL	GOx in reduced form 	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evaluation of an electron-transfer mediator useful for glucose oxidation is discussed from thermodynamic and kinetic points of view , i.e. the redox potentials of various metal complexes and the second-order rate constants for the electron transfer between GOx in reduced form and the metal complexes in oxidized form .
	manualset3
151309	11	409919	7	NULL	NULL	NULL	NULL	metal complexes in oxidized form	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evaluation of an electron-transfer mediator useful for glucose oxidation is discussed from thermodynamic and kinetic points of view , i.e. the redox potentials of various metal complexes and the second-order rate constants for the electron transfer between GOx in reduced form and the metal complexes in oxidized form .
	manualset3
151318	1	409920	7	NULL	NULL	0	NULL	evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of mineralized collagen as a carrier for the osteoinductive material COLLOSS ( ) E , in vivo .
	manualset3
151321	2	409920	7	NULL	NULL	0	NULL	mineralized collagen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of mineralized collagen as a carrier for the osteoinductive material COLLOSS ( ) E , in vivo .
	manualset3
151327	3	409920	7	NULL	NULL	0	NULL	carrier	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of mineralized collagen as a carrier for the osteoinductive material COLLOSS ( ) E , in vivo .
	manualset3
151332	4	409920	7	NULL	NULL	0	NULL	osteoinductive material 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of mineralized collagen as a carrier for the osteoinductive material COLLOSS ( ) E , in vivo .
	manualset3
151334	5	409920	7	NULL	NULL	0	NULL	COLLOSS ( ) E	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of mineralized collagen as a carrier for the osteoinductive material COLLOSS ( ) E , in vivo .
	manualset3
151336	6	409920	7	NULL	NULL	0	NULL	in vivo	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of mineralized collagen as a carrier for the osteoinductive material COLLOSS ( ) E , in vivo .
	manualset3
151368	1	409921	7	NULL	NULL	0	NULL	evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of the effect of artefact suppression on those channels close to the eyes was compared with standard ordinary least squares method ( OLS ) based on a linear model of the influence of EOG on ERP .
	manualset3
151369	2	409921	7	NULL	NULL	0	NULL	effect of artefact suppression	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of the effect of artefact suppression on those channels close to the eyes was compared with standard ordinary least squares method ( OLS ) based on a linear model of the influence of EOG on ERP .
	manualset3
151370	3	409921	7	NULL	NULL	NULL	NULL	channels	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evaluation of the effect of artefact suppression on those channels close to the eyes was compared with standard ordinary least squares method ( OLS ) based on a linear model of the influence of EOG on ERP .
	manualset3
151371	4	409921	7	NULL	NULL	0	NULL	eyes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of the effect of artefact suppression on those channels close to the eyes was compared with standard ordinary least squares method ( OLS ) based on a linear model of the influence of EOG on ERP .
	manualset3
151372	5	409921	7	NULL	NULL	NULL	NULL	standard ordinary least squares method ( OLS )	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evaluation of the effect of artefact suppression on those channels close to the eyes was compared with standard ordinary least squares method ( OLS ) based on a linear model of the influence of EOG on ERP .
	manualset3
151373	6	409921	7	NULL	NULL	NULL	NULL	linear model 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evaluation of the effect of artefact suppression on those channels close to the eyes was compared with standard ordinary least squares method ( OLS ) based on a linear model of the influence of EOG on ERP .
	manualset3
151374	7	409921	7	NULL	NULL	NULL	NULL	 EOG	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evaluation of the effect of artefact suppression on those channels close to the eyes was compared with standard ordinary least squares method ( OLS ) based on a linear model of the influence of EOG on ERP .
	manualset3
151375	8	409921	7	NULL	NULL	0	NULL	ERP	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of the effect of artefact suppression on those channels close to the eyes was compared with standard ordinary least squares method ( OLS ) based on a linear model of the influence of EOG on ERP .
	manualset3
151376	1	409922	7	NULL	NULL	0	NULL	evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of the specificity and the affinity constants of the antiserum is studied by radioimmunoassay against different antiepileptic drugs and metallotracers ( phenytoin labeled with organometallic fragments derived respectively from cobaltocene and ferrocene ) .
	manualset3
151377	2	409922	7	NULL	NULL	0	NULL	specificity constant	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of the specificity and the affinity constants of the antiserum is studied by radioimmunoassay against different antiepileptic drugs and metallotracers ( phenytoin labeled with organometallic fragments derived respectively from cobaltocene and ferrocene ) .
	manualset3
151378	3	409922	7	NULL	NULL	0	NULL	affinity constants	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of the specificity and the affinity constants of the antiserum is studied by radioimmunoassay against different antiepileptic drugs and metallotracers ( phenytoin labeled with organometallic fragments derived respectively from cobaltocene and ferrocene ) .
	manualset3
151379	4	409922	7	NULL	NULL	NULL	NULL	antiserum	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evaluation of the specificity and the affinity constants of the antiserum is studied by radioimmunoassay against different antiepileptic drugs and metallotracers ( phenytoin labeled with organometallic fragments derived respectively from cobaltocene and ferrocene ) .
	manualset3
151380	5	409922	7	NULL	NULL	0	NULL	radioimmunoassay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of the specificity and the affinity constants of the antiserum is studied by radioimmunoassay against different antiepileptic drugs and metallotracers ( phenytoin labeled with organometallic fragments derived respectively from cobaltocene and ferrocene ) .
	manualset3
151381	6	409922	7	NULL	NULL	0	NULL	antiepileptic drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of the specificity and the affinity constants of the antiserum is studied by radioimmunoassay against different antiepileptic drugs and metallotracers ( phenytoin labeled with organometallic fragments derived respectively from cobaltocene and ferrocene ) .
	manualset3
151382	7	409922	7	NULL	NULL	0	NULL	metallotracers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of the specificity and the affinity constants of the antiserum is studied by radioimmunoassay against different antiepileptic drugs and metallotracers ( phenytoin labeled with organometallic fragments derived respectively from cobaltocene and ferrocene ) .
	manualset3
151383	8	409922	7	NULL	NULL	0	NULL	 phenytoin labeled with organometallic fragments	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of the specificity and the affinity constants of the antiserum is studied by radioimmunoassay against different antiepileptic drugs and metallotracers ( phenytoin labeled with organometallic fragments derived respectively from cobaltocene and ferrocene ) .
	manualset3
151384	9	409922	7	NULL	NULL	0	NULL	 cobaltocene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of the specificity and the affinity constants of the antiserum is studied by radioimmunoassay against different antiepileptic drugs and metallotracers ( phenytoin labeled with organometallic fragments derived respectively from cobaltocene and ferrocene ) .
	manualset3
151385	10	409922	7	NULL	NULL	0	NULL	ferrocene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of the specificity and the affinity constants of the antiserum is studied by radioimmunoassay against different antiepileptic drugs and metallotracers ( phenytoin labeled with organometallic fragments derived respectively from cobaltocene and ferrocene ) .
	manualset3
151386	1	409923	7	NULL	NULL	0	NULL	evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of the structure of the spongious substance of the tibiotarsal ( TT ) bones of the domestic duck aged 4 to 8 wk was performed using radiological analysis .
	manualset3
151387	2	409923	7	NULL	NULL	0	NULL	structure	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of the structure of the spongious substance of the tibiotarsal ( TT ) bones of the domestic duck aged 4 to 8 wk was performed using radiological analysis .
	manualset3
151388	3	409923	7	NULL	NULL	0	NULL	spongious substance of the tibiotarsal ( TT ) bones	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of the structure of the spongious substance of the tibiotarsal ( TT ) bones of the domestic duck aged 4 to 8 wk was performed using radiological analysis .
	manualset3
151389	4	409923	7	NULL	NULL	0	NULL	domestic duck	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of the structure of the spongious substance of the tibiotarsal ( TT ) bones of the domestic duck aged 4 to 8 wk was performed using radiological analysis .
	manualset3
151390	5	409923	7	NULL	NULL	0	NULL	4 to 8 wk	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of the structure of the spongious substance of the tibiotarsal ( TT ) bones of the domestic duck aged 4 to 8 wk was performed using radiological analysis .
	manualset3
151391	6	409923	7	NULL	NULL	0	NULL	radiological analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of the structure of the spongious substance of the tibiotarsal ( TT ) bones of the domestic duck aged 4 to 8 wk was performed using radiological analysis .
	manualset3
151392	1	409924	7	NULL	NULL	0	NULL	event	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The event has since been discontinued .
	manualset3
151394	1	409925	7	NULL	NULL	0	NULL	events	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The events induced by bradykinin were accompanied by an increase in the intracellular calcium concentration , as monitored by quin-2 fluorescence .
	manualset3
151395	2	409925	7	NULL	NULL	0	NULL	bradykinin	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The events induced by bradykinin were accompanied by an increase in the intracellular calcium concentration , as monitored by quin-2 fluorescence .
	manualset3
151396	3	409925	7	NULL	NULL	0	NULL	intracellular calcium concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The events induced by bradykinin were accompanied by an increase in the intracellular calcium concentration , as monitored by quin-2 fluorescence .
	manualset3
151397	4	409925	7	NULL	NULL	0	NULL	quin-2 fluorescence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The events induced by bradykinin were accompanied by an increase in the intracellular calcium concentration , as monitored by quin-2 fluorescence .
	manualset3
151460	1	409926	7	NULL	NULL	NULL	NULL	eventual pregnancy rate	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The eventual pregnancy rate after unilateral salpingostomy with bilateral division of adhesions ( 43.8 % ; n = 16 ) , however , was comparable to that after bilateral salpingolysis for purely peritubal adhesions ( 54.1 % n = 37 ) .
	manualset3
151464	2	409926	7	NULL	NULL	0	NULL	unilateral salpingostomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The eventual pregnancy rate after unilateral salpingostomy with bilateral division of adhesions ( 43.8 % ; n = 16 ) , however , was comparable to that after bilateral salpingolysis for purely peritubal adhesions ( 54.1 % n = 37 ) .
	manualset3
151467	3	409926	7	NULL	NULL	NULL	NULL	bilateral division of adhesions	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The eventual pregnancy rate after unilateral salpingostomy with bilateral division of adhesions ( 43.8 % ; n = 16 ) , however , was comparable to that after bilateral salpingolysis for purely peritubal adhesions ( 54.1 % n = 37 ) .
	manualset3
151471	4	409926	7	NULL	NULL	0	NULL	43.8 % ; n = 16	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The eventual pregnancy rate after unilateral salpingostomy with bilateral division of adhesions ( 43.8 % ; n = 16 ) , however , was comparable to that after bilateral salpingolysis for purely peritubal adhesions ( 54.1 % n = 37 ) .
	manualset3
151472	5	409926	7	NULL	NULL	0	NULL	bilateral salpingolysis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The eventual pregnancy rate after unilateral salpingostomy with bilateral division of adhesions ( 43.8 % ; n = 16 ) , however , was comparable to that after bilateral salpingolysis for purely peritubal adhesions ( 54.1 % n = 37 ) .
	manualset3
151473	6	409926	7	NULL	NULL	NULL	NULL	purely peritubal adhesions	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The eventual pregnancy rate after unilateral salpingostomy with bilateral division of adhesions ( 43.8 % ; n = 16 ) , however , was comparable to that after bilateral salpingolysis for purely peritubal adhesions ( 54.1 % n = 37 ) .
	manualset3
151485	7	409926	7	NULL	NULL	0	NULL	54.1 % n = 37	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The eventual pregnancy rate after unilateral salpingostomy with bilateral division of adhesions ( 43.8 % ; n = 16 ) , however , was comparable to that after bilateral salpingolysis for purely peritubal adhesions ( 54.1 % n = 37 ) .
	manualset3
151496	1	409927	7	NULL	NULL	NULL	NULL	evidence	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evidence currently available emphasizes the importance of diffuse damage in closed head injury .
	manualset3
151499	2	409927	7	NULL	NULL	NULL	NULL	currently available	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evidence currently available emphasizes the importance of diffuse damage in closed head injury .
	manualset3
151511	3	409927	7	NULL	NULL	0	NULL	diffuse damage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The evidence currently available emphasizes the importance of diffuse damage in closed head injury .
	manualset3
151513	4	409927	7	NULL	NULL	NULL	NULL	closed head injury	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evidence currently available emphasizes the importance of diffuse damage in closed head injury .
	manualset3
151525	1	409928	7	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The evidence for the presence of tIssue-specific localization of p38CTBP has indicated that p38CTBP has a tIssue-specific function , such as the regulation of T3 delivery from cytoplasm to nuclei .
	manualset3
151526	2	409928	7	NULL	NULL	0	NULL	tIssue-specific localization	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The evidence for the presence of tIssue-specific localization of p38CTBP has indicated that p38CTBP has a tIssue-specific function , such as the regulation of T3 delivery from cytoplasm to nuclei .
	manualset3
151530	3	409928	7	NULL	NULL	0	NULL	p38CTBP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The evidence for the presence of tIssue-specific localization of p38CTBP has indicated that p38CTBP has a tIssue-specific function , such as the regulation of T3 delivery from cytoplasm to nuclei .
	manualset3
151535	4	409928	7	NULL	NULL	0	NULL	tIssue-specific function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The evidence for the presence of tIssue-specific localization of p38CTBP has indicated that p38CTBP has a tIssue-specific function , such as the regulation of T3 delivery from cytoplasm to nuclei .
	manualset3
151536	5	409928	7	NULL	NULL	NULL	NULL	regulation of T3 delivery	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evidence for the presence of tIssue-specific localization of p38CTBP has indicated that p38CTBP has a tIssue-specific function , such as the regulation of T3 delivery from cytoplasm to nuclei .
	manualset3
151540	6	409928	7	NULL	NULL	NULL	NULL	cytoplasm	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evidence for the presence of tIssue-specific localization of p38CTBP has indicated that p38CTBP has a tIssue-specific function , such as the regulation of T3 delivery from cytoplasm to nuclei .
	manualset3
151541	7	409928	7	NULL	NULL	NULL	NULL	nuclei	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evidence for the presence of tIssue-specific localization of p38CTBP has indicated that p38CTBP has a tIssue-specific function , such as the regulation of T3 delivery from cytoplasm to nuclei .
	manualset3
151603	1	409929	7	NULL	NULL	NULL	NULL	evidence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evidence for their impact on return-to-work is examined within the framework of the Phase Model of Disability , which puts forth the phase-specificity of symptoms , risks , and interventions for disability .
	manualset3
151604	2	409929	7	NULL	NULL	NULL	NULL	return-to-work	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evidence for their impact on return-to-work is examined within the framework of the Phase Model of Disability , which puts forth the phase-specificity of symptoms , risks , and interventions for disability .
	manualset3
151605	3	409929	7	NULL	NULL	0	NULL	framework	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The evidence for their impact on return-to-work is examined within the framework of the Phase Model of Disability , which puts forth the phase-specificity of symptoms , risks , and interventions for disability .
	manualset3
151606	4	409929	7	NULL	NULL	NULL	NULL	Phase Model of Disability	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evidence for their impact on return-to-work is examined within the framework of the Phase Model of Disability , which puts forth the phase-specificity of symptoms , risks , and interventions for disability .
	manualset3
151607	5	409929	7	NULL	NULL	NULL	NULL	phase-specificity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evidence for their impact on return-to-work is examined within the framework of the Phase Model of Disability , which puts forth the phase-specificity of symptoms , risks , and interventions for disability .
	manualset3
151608	6	409929	7	NULL	NULL	0	NULL	symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The evidence for their impact on return-to-work is examined within the framework of the Phase Model of Disability , which puts forth the phase-specificity of symptoms , risks , and interventions for disability .
	manualset3
151609	7	409929	7	NULL	NULL	0	NULL	risks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The evidence for their impact on return-to-work is examined within the framework of the Phase Model of Disability , which puts forth the phase-specificity of symptoms , risks , and interventions for disability .
	manualset3
151610	8	409929	7	NULL	NULL	0	NULL	interventions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The evidence for their impact on return-to-work is examined within the framework of the Phase Model of Disability , which puts forth the phase-specificity of symptoms , risks , and interventions for disability .
	manualset3
151611	9	409929	7	NULL	NULL	0	NULL	disability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The evidence for their impact on return-to-work is examined within the framework of the Phase Model of Disability , which puts forth the phase-specificity of symptoms , risks , and interventions for disability .
	manualset3
151612	1	409930	7	NULL	NULL	0	NULL	evidence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The evidence that BglM1 localizes on the plasma membrane of plasmodia was confirmed using immunofluorescence microscopy .
	manualset3
151613	2	409930	7	NULL	NULL	0	NULL	BglM1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The evidence that BglM1 localizes on the plasma membrane of plasmodia was confirmed using immunofluorescence microscopy .
	manualset3
151614	3	409930	7	NULL	NULL	0	NULL	plasma membrane 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The evidence that BglM1 localizes on the plasma membrane of plasmodia was confirmed using immunofluorescence microscopy .
	manualset3
151615	4	409930	7	NULL	NULL	0	NULL	plasmodia	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The evidence that BglM1 localizes on the plasma membrane of plasmodia was confirmed using immunofluorescence microscopy .
	manualset3
151616	5	409930	7	NULL	NULL	0	NULL	 immunofluorescence microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The evidence that BglM1 localizes on the plasma membrane of plasmodia was confirmed using immunofluorescence microscopy .
	manualset3
151722	1	409931	7	NULL	NULL	NULL	NULL	evoked expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evoked expression of the immediate early gene ( IEG ) - encoded proteins c-Fos and Krox-24 was used to monitor spinal visceronociceptive processing that results from cyclophosphamide cystitis in behaving rats .
	manualset3
151727	2	409931	7	NULL	NULL	NULL	NULL	 immediate early gene ( IEG ) encoded proteins	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evoked expression of the immediate early gene ( IEG ) - encoded proteins c-Fos and Krox-24 was used to monitor spinal visceronociceptive processing that results from cyclophosphamide cystitis in behaving rats .
	manualset3
151732	3	409931	7	NULL	NULL	NULL	NULL	 c-Fos 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evoked expression of the immediate early gene ( IEG ) - encoded proteins c-Fos and Krox-24 was used to monitor spinal visceronociceptive processing that results from cyclophosphamide cystitis in behaving rats .
	manualset3
151733	4	409931	7	NULL	NULL	NULL	NULL	Krox-24	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evoked expression of the immediate early gene ( IEG ) - encoded proteins c-Fos and Krox-24 was used to monitor spinal visceronociceptive processing that results from cyclophosphamide cystitis in behaving rats .
	manualset3
151734	5	409931	7	NULL	NULL	0	NULL	spinal visceronociceptive processing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The evoked expression of the immediate early gene ( IEG ) - encoded proteins c-Fos and Krox-24 was used to monitor spinal visceronociceptive processing that results from cyclophosphamide cystitis in behaving rats .
	manualset3
151735	6	409931	7	NULL	NULL	0	NULL	cyclophosphamide cystitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The evoked expression of the immediate early gene ( IEG ) - encoded proteins c-Fos and Krox-24 was used to monitor spinal visceronociceptive processing that results from cyclophosphamide cystitis in behaving rats .
	manualset3
151736	7	409931	7	NULL	NULL	NULL	NULL	 rats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evoked expression of the immediate early gene ( IEG ) - encoded proteins c-Fos and Krox-24 was used to monitor spinal visceronociceptive processing that results from cyclophosphamide cystitis in behaving rats .
	manualset3
151737	1	409932	7	NULL	NULL	0	NULL	evolution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The evolution and treatment response suggests that at least in some cases of the Landau-Kleffner syndrome , the etiology of the aphasia and other neuropsychological deficits and of the behavior disorders are related with some subclinical epileptic discharges and with a `` functional inhibition '' of some areas of the nervous system .
	manualset3
151738	2	409932	7	NULL	NULL	0	NULL	 treatment response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The evolution and treatment response suggests that at least in some cases of the Landau-Kleffner syndrome , the etiology of the aphasia and other neuropsychological deficits and of the behavior disorders are related with some subclinical epileptic discharges and with a `` functional inhibition '' of some areas of the nervous system .
	manualset3
151739	3	409932	7	NULL	NULL	0	NULL	Landau-Kleffner syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The evolution and treatment response suggests that at least in some cases of the Landau-Kleffner syndrome , the etiology of the aphasia and other neuropsychological deficits and of the behavior disorders are related with some subclinical epileptic discharges and with a `` functional inhibition '' of some areas of the nervous system .
	manualset3
151740	4	409932	7	NULL	NULL	NULL	NULL	etiology 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evolution and treatment response suggests that at least in some cases of the Landau-Kleffner syndrome , the etiology of the aphasia and other neuropsychological deficits and of the behavior disorders are related with some subclinical epileptic discharges and with a `` functional inhibition '' of some areas of the nervous system .
	manualset3
151741	6	409932	7	NULL	NULL	NULL	NULL	neuropsychological deficits	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evolution and treatment response suggests that at least in some cases of the Landau-Kleffner syndrome , the etiology of the aphasia and other neuropsychological deficits and of the behavior disorders are related with some subclinical epileptic discharges and with a `` functional inhibition '' of some areas of the nervous system .
	manualset3
151742	7	409932	7	NULL	NULL	NULL	NULL	behavior disorders	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evolution and treatment response suggests that at least in some cases of the Landau-Kleffner syndrome , the etiology of the aphasia and other neuropsychological deficits and of the behavior disorders are related with some subclinical epileptic discharges and with a `` functional inhibition '' of some areas of the nervous system .
	manualset3
151743	8	409932	7	NULL	NULL	NULL	NULL	subclinical epileptic discharges	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evolution and treatment response suggests that at least in some cases of the Landau-Kleffner syndrome , the etiology of the aphasia and other neuropsychological deficits and of the behavior disorders are related with some subclinical epileptic discharges and with a `` functional inhibition '' of some areas of the nervous system .
	manualset3
151744	9	409932	7	NULL	NULL	NULL	NULL	functional inhibition	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evolution and treatment response suggests that at least in some cases of the Landau-Kleffner syndrome , the etiology of the aphasia and other neuropsychological deficits and of the behavior disorders are related with some subclinical epileptic discharges and with a `` functional inhibition '' of some areas of the nervous system .
	manualset3
151745	10	409932	7	NULL	NULL	NULL	NULL	nervous system	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evolution and treatment response suggests that at least in some cases of the Landau-Kleffner syndrome , the etiology of the aphasia and other neuropsychological deficits and of the behavior disorders are related with some subclinical epileptic discharges and with a `` functional inhibition '' of some areas of the nervous system .
	manualset3
153351	5	409932	7	NULL	NULL	0	NULL	aphasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The evolution and treatment response suggests that at least in some cases of the Landau-Kleffner syndrome , the etiology of the aphasia and other neuropsychological deficits and of the behavior disorders are related with some subclinical epileptic discharges and with a `` functional inhibition '' of some areas of the nervous system .
	manualset3
151746	1	409933	7	NULL	NULL	NULL	NULL	evolution	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evolution of the dislocation structure that forms during uniaxial creep deformation in the single-crystal superalloy LEK94 of low density and with Re additions was analyzed using transmission electron microscopy .
	manualset3
151756	2	409933	7	NULL	NULL	0	NULL	dislocation structure	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The evolution of the dislocation structure that forms during uniaxial creep deformation in the single-crystal superalloy LEK94 of low density and with Re additions was analyzed using transmission electron microscopy .
	manualset3
151767	3	409933	7	NULL	NULL	0	NULL	uniaxial creep deformation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The evolution of the dislocation structure that forms during uniaxial creep deformation in the single-crystal superalloy LEK94 of low density and with Re additions was analyzed using transmission electron microscopy .
	manualset3
151770	4	409933	7	NULL	NULL	0	NULL	single-crystal superalloy LEK94	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The evolution of the dislocation structure that forms during uniaxial creep deformation in the single-crystal superalloy LEK94 of low density and with Re additions was analyzed using transmission electron microscopy .
	manualset3
151771	5	409933	7	NULL	NULL	0	NULL	low density	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The evolution of the dislocation structure that forms during uniaxial creep deformation in the single-crystal superalloy LEK94 of low density and with Re additions was analyzed using transmission electron microscopy .
	manualset3
151772	6	409933	7	NULL	NULL	0	NULL	Re additions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The evolution of the dislocation structure that forms during uniaxial creep deformation in the single-crystal superalloy LEK94 of low density and with Re additions was analyzed using transmission electron microscopy .
	manualset3
151773	7	409933	7	NULL	NULL	0	NULL	transmission electron microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The evolution of the dislocation structure that forms during uniaxial creep deformation in the single-crystal superalloy LEK94 of low density and with Re additions was analyzed using transmission electron microscopy .
	manualset3
151777	1	409934	7	NULL	NULL	0	NULL	evolutionary dynamics 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The evolutionary dynamics of HIV during the chronic phase of infection is driven by the host immune response and by selective pressures exerted through drug treatment .
	manualset3
151781	2	409934	7	NULL	NULL	0	NULL	HIV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The evolutionary dynamics of HIV during the chronic phase of infection is driven by the host immune response and by selective pressures exerted through drug treatment .
	manualset3
151782	3	409934	7	NULL	NULL	0	NULL	chronic phase of infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The evolutionary dynamics of HIV during the chronic phase of infection is driven by the host immune response and by selective pressures exerted through drug treatment .
	manualset3
151783	4	409934	7	NULL	NULL	0	NULL	host immune response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The evolutionary dynamics of HIV during the chronic phase of infection is driven by the host immune response and by selective pressures exerted through drug treatment .
	manualset3
151784	5	409934	7	NULL	NULL	0	NULL	selective pressures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The evolutionary dynamics of HIV during the chronic phase of infection is driven by the host immune response and by selective pressures exerted through drug treatment .
	manualset3
151785	6	409934	7	NULL	NULL	0	NULL	drug treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The evolutionary dynamics of HIV during the chronic phase of infection is driven by the host immune response and by selective pressures exerted through drug treatment .
	manualset3
151786	1	409935	7	NULL	NULL	NULL	NULL	evolutionary fate	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evolutionary fate and consequences of duplicate genes .
	manualset3
151788	2	409935	7	NULL	NULL	NULL	NULL	duplicate genes	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evolutionary fate and consequences of duplicate genes .
	manualset3
151789	1	409936	7	NULL	NULL	NULL	NULL	molecular basis	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The exact molecular basis of tigecycline action is not clear at present , although similarly to the tetracyclines , it has been shown to inhibit the translation elongation step by binding to the ribosome 30S subunit and preventing aminoacylated tRNAs to accommodate in the ribosomal A site .
	manualset3
151790	2	409936	7	NULL	NULL	NULL	NULL	tigecycline action	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The exact molecular basis of tigecycline action is not clear at present , although similarly to the tetracyclines , it has been shown to inhibit the translation elongation step by binding to the ribosome 30S subunit and preventing aminoacylated tRNAs to accommodate in the ribosomal A site .
	manualset3
151791	3	409936	7	NULL	NULL	0	NULL	tetracyclines	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The exact molecular basis of tigecycline action is not clear at present , although similarly to the tetracyclines , it has been shown to inhibit the translation elongation step by binding to the ribosome 30S subunit and preventing aminoacylated tRNAs to accommodate in the ribosomal A site .
	manualset3
151793	4	409936	7	NULL	NULL	NULL	NULL	translation elongation step	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The exact molecular basis of tigecycline action is not clear at present , although similarly to the tetracyclines , it has been shown to inhibit the translation elongation step by binding to the ribosome 30S subunit and preventing aminoacylated tRNAs to accommodate in the ribosomal A site .
	manualset3
151794	5	409936	7	NULL	NULL	NULL	NULL	ribosome 30S subunit	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The exact molecular basis of tigecycline action is not clear at present , although similarly to the tetracyclines , it has been shown to inhibit the translation elongation step by binding to the ribosome 30S subunit and preventing aminoacylated tRNAs to accommodate in the ribosomal A site .
	manualset3
151795	6	409936	7	NULL	NULL	NULL	NULL	aminoacylated tRNAs	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The exact molecular basis of tigecycline action is not clear at present , although similarly to the tetracyclines , it has been shown to inhibit the translation elongation step by binding to the ribosome 30S subunit and preventing aminoacylated tRNAs to accommodate in the ribosomal A site .
	manualset3
151796	7	409936	7	NULL	NULL	NULL	NULL	ribosomal A site	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The exact molecular basis of tigecycline action is not clear at present , although similarly to the tetracyclines , it has been shown to inhibit the translation elongation step by binding to the ribosome 30S subunit and preventing aminoacylated tRNAs to accommodate in the ribosomal A site .
	manualset3
151797	1	409937	7	NULL	NULL	0	NULL	example	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The example of metabolic susceptibility to cancer .
	manualset3
151798	2	409937	7	NULL	NULL	NULL	NULL	metabolic susceptibility	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The example of metabolic susceptibility to cancer .
	manualset3
151799	3	409937	7	NULL	NULL	NULL	NULL	cancer	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The example of metabolic susceptibility to cancer .
	manualset3
151825	1	409938	7	NULL	NULL	0	NULL	excellent agreement	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The excellent agreement of the simulated with the experimental spectra allows an assignment of the observed peaks in the sum frequency spectra of the water/corundum ( 0001 ) interface on the basis of our theoretical data .
	manualset3
151826	3	409938	7	NULL	NULL	NULL	NULL	experimental spectra	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The excellent agreement of the simulated with the experimental spectra allows an assignment of the observed peaks in the sum frequency spectra of the water/corundum ( 0001 ) interface on the basis of our theoretical data .
	manualset3
151828	4	409938	7	NULL	NULL	0	NULL	assignment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The excellent agreement of the simulated with the experimental spectra allows an assignment of the observed peaks in the sum frequency spectra of the water/corundum ( 0001 ) interface on the basis of our theoretical data .
	manualset3
151829	5	409938	7	NULL	NULL	NULL	NULL	observed peaks	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The excellent agreement of the simulated with the experimental spectra allows an assignment of the observed peaks in the sum frequency spectra of the water/corundum ( 0001 ) interface on the basis of our theoretical data .
	manualset3
151830	6	409938	7	NULL	NULL	0	NULL	sum frequency spectra	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The excellent agreement of the simulated with the experimental spectra allows an assignment of the observed peaks in the sum frequency spectra of the water/corundum ( 0001 ) interface on the basis of our theoretical data .
	manualset3
151831	7	409938	7	NULL	NULL	0	NULL	water/corundum ( 0001 ) interface	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The excellent agreement of the simulated with the experimental spectra allows an assignment of the observed peaks in the sum frequency spectra of the water/corundum ( 0001 ) interface on the basis of our theoretical data .
	manualset3
151832	8	409938	7	NULL	NULL	NULL	NULL	theoretical data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The excellent agreement of the simulated with the experimental spectra allows an assignment of the observed peaks in the sum frequency spectra of the water/corundum ( 0001 ) interface on the basis of our theoretical data .
	manualset3
151833	1	409939	7	NULL	NULL	0	NULL	exception 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The exception to this was that the incidence of abnormal sural nerve SEPs decreased postoperatively .
	manualset3
151834	2	409939	7	NULL	NULL	0	NULL	incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The exception to this was that the incidence of abnormal sural nerve SEPs decreased postoperatively .
	manualset3
151835	3	409939	7	NULL	NULL	0	NULL	abnormal sural nerve SEPs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The exception to this was that the incidence of abnormal sural nerve SEPs decreased postoperatively .
	manualset3
151836	4	409939	7	NULL	NULL	0	NULL	postoperatively	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The exception to this was that the incidence of abnormal sural nerve SEPs decreased postoperatively .
	manualset3
151837	1	409940	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A study of the teaching and learning of the biological sciences in nurse education .
	manualset3
151838	2	409940	7	NULL	NULL	NULL	NULL	teaching	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A study of the teaching and learning of the biological sciences in nurse education .
	manualset3
151839	3	409940	7	NULL	NULL	NULL	NULL	learning	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A study of the teaching and learning of the biological sciences in nurse education .
	manualset3
151840	4	409940	7	NULL	NULL	0	NULL	biological sciences	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A study of the teaching and learning of the biological sciences in nurse education .
	manualset3
151841	5	409940	7	NULL	NULL	0	NULL	nurse education	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A study of the teaching and learning of the biological sciences in nurse education .
	manualset3
151975	1	409941	7	NULL	NULL	NULL	NULL	excited states	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The excited states were characterized quantitatively by time-correlated single photon counting , femtosecond transient absorption spectroscopy , and nanosecond laser flash photolysis .
	manualset3
151977	2	409941	7	NULL	NULL	NULL	NULL	time-correlated single photon counting	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The excited states were characterized quantitatively by time-correlated single photon counting , femtosecond transient absorption spectroscopy , and nanosecond laser flash photolysis .
	manualset3
151978	3	409941	7	NULL	NULL	NULL	NULL	femtosecond transient absorption spectroscopy	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The excited states were characterized quantitatively by time-correlated single photon counting , femtosecond transient absorption spectroscopy , and nanosecond laser flash photolysis .
	manualset3
151981	4	409941	7	NULL	NULL	NULL	NULL	nanosecond laser flash photolysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The excited states were characterized quantitatively by time-correlated single photon counting , femtosecond transient absorption spectroscopy , and nanosecond laser flash photolysis .
	manualset3
151996	1	409942	7	NULL	NULL	0	NULL	existence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The existence of an energy barrier upon entry to the molten globule is examined as well .
	manualset3
151998	2	409942	7	NULL	NULL	0	NULL	energy barrier	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The existence of an energy barrier upon entry to the molten globule is examined as well .
	manualset3
152007	3	409942	7	NULL	NULL	0	NULL	molten globule	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The existence of an energy barrier upon entry to the molten globule is examined as well .
	manualset3
152008	1	409943	7	NULL	NULL	0	NULL	exonuclease activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The exonuclease activity associated with DNA polymerase delta removes araCMP from 3 ' termini with the same efficiency that it removes a paired 3 ' deoxycytosine suggesting that the proofreading exonucleases associated with DNA polymerases might remove aranucleotides inefficiently .
	manualset3
152009	2	409943	7	NULL	NULL	0	NULL	DNA polymerase delta 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The exonuclease activity associated with DNA polymerase delta removes araCMP from 3 ' termini with the same efficiency that it removes a paired 3 ' deoxycytosine suggesting that the proofreading exonucleases associated with DNA polymerases might remove aranucleotides inefficiently .
	manualset3
152010	3	409943	7	NULL	NULL	0	NULL	araCMP 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The exonuclease activity associated with DNA polymerase delta removes araCMP from 3 ' termini with the same efficiency that it removes a paired 3 ' deoxycytosine suggesting that the proofreading exonucleases associated with DNA polymerases might remove aranucleotides inefficiently .
	manualset3
152015	4	409943	7	NULL	NULL	0	NULL	3 ' termini	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The exonuclease activity associated with DNA polymerase delta removes araCMP from 3 ' termini with the same efficiency that it removes a paired 3 ' deoxycytosine suggesting that the proofreading exonucleases associated with DNA polymerases might remove aranucleotides inefficiently .
	manualset3
152016	5	409943	7	NULL	NULL	0	NULL	same efficiency	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The exonuclease activity associated with DNA polymerase delta removes araCMP from 3 ' termini with the same efficiency that it removes a paired 3 ' deoxycytosine suggesting that the proofreading exonucleases associated with DNA polymerases might remove aranucleotides inefficiently .
	manualset3
152020	6	409943	7	NULL	NULL	0	NULL	paired 3 ' deoxycytosine	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The exonuclease activity associated with DNA polymerase delta removes araCMP from 3 ' termini with the same efficiency that it removes a paired 3 ' deoxycytosine suggesting that the proofreading exonucleases associated with DNA polymerases might remove aranucleotides inefficiently .
	manualset3
152024	7	409943	7	NULL	NULL	0	NULL	proofreading exonucleases	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The exonuclease activity associated with DNA polymerase delta removes araCMP from 3 ' termini with the same efficiency that it removes a paired 3 ' deoxycytosine suggesting that the proofreading exonucleases associated with DNA polymerases might remove aranucleotides inefficiently .
	manualset3
152025	8	409943	7	NULL	NULL	0	NULL	DNA polymerases 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The exonuclease activity associated with DNA polymerase delta removes araCMP from 3 ' termini with the same efficiency that it removes a paired 3 ' deoxycytosine suggesting that the proofreading exonucleases associated with DNA polymerases might remove aranucleotides inefficiently .
	manualset3
152029	10	409943	7	NULL	NULL	0	NULL	aranucleotides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The exonuclease activity associated with DNA polymerase delta removes araCMP from 3 ' termini with the same efficiency that it removes a paired 3 ' deoxycytosine suggesting that the proofreading exonucleases associated with DNA polymerases might remove aranucleotides inefficiently .
	manualset3
152045	1	409944	7	NULL	NULL	0	NULL	expanded NKG2C ( + ) NK cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The expanded NKG2C ( + ) NK cells display a terminally differentiated phenotype with strong functional responses against HLA-E-expressing targets and antibody-coated targets but not to IL-12 / IL-18 stimulation .
	manualset3
152046	2	409944	7	NULL	NULL	NULL	NULL	phenotype	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expanded NKG2C ( + ) NK cells display a terminally differentiated phenotype with strong functional responses against HLA-E-expressing targets and antibody-coated targets but not to IL-12 / IL-18 stimulation .
	manualset3
152057	4	409944	7	NULL	NULL	0	NULL	strong functional responses	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The expanded NKG2C ( + ) NK cells display a terminally differentiated phenotype with strong functional responses against HLA-E-expressing targets and antibody-coated targets but not to IL-12 / IL-18 stimulation .
	manualset3
152060	5	409944	7	NULL	NULL	NULL	NULL	HLA-E-expressing targets	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expanded NKG2C ( + ) NK cells display a terminally differentiated phenotype with strong functional responses against HLA-E-expressing targets and antibody-coated targets but not to IL-12 / IL-18 stimulation .
	manualset3
152066	6	409944	7	NULL	NULL	0	NULL	antibody-coated targets	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The expanded NKG2C ( + ) NK cells display a terminally differentiated phenotype with strong functional responses against HLA-E-expressing targets and antibody-coated targets but not to IL-12 / IL-18 stimulation .
	manualset3
152070	7	409944	7	NULL	NULL	0	NULL	IL-12  stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The expanded NKG2C ( + ) NK cells display a terminally differentiated phenotype with strong functional responses against HLA-E-expressing targets and antibody-coated targets but not to IL-12 / IL-18 stimulation .
	manualset3
152072	8	409944	7	NULL	NULL	0	NULL	IL-18 stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The expanded NKG2C ( + ) NK cells display a terminally differentiated phenotype with strong functional responses against HLA-E-expressing targets and antibody-coated targets but not to IL-12 / IL-18 stimulation .
	manualset3
152082	1	409945	7	NULL	NULL	0	NULL	expected overall life-years ( LYs ) 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The expected overall life-years ( LYs ) obtained were 3.68 years for letrozole arm and 3.09 years for tamoxifen arm , showing incremental LYs of 0.59 years in patients receiving letrozole .
	manualset3
152086	2	409945	7	NULL	NULL	0	NULL	3.68 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The expected overall life-years ( LYs ) obtained were 3.68 years for letrozole arm and 3.09 years for tamoxifen arm , showing incremental LYs of 0.59 years in patients receiving letrozole .
	manualset3
152087	3	409945	7	NULL	NULL	0	NULL	letrozole arm	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The expected overall life-years ( LYs ) obtained were 3.68 years for letrozole arm and 3.09 years for tamoxifen arm , showing incremental LYs of 0.59 years in patients receiving letrozole .
	manualset3
152089	4	409945	7	NULL	NULL	0	NULL	3.09 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The expected overall life-years ( LYs ) obtained were 3.68 years for letrozole arm and 3.09 years for tamoxifen arm , showing incremental LYs of 0.59 years in patients receiving letrozole .
	manualset3
152091	5	409945	7	NULL	NULL	0	NULL	tamoxifen arm	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The expected overall life-years ( LYs ) obtained were 3.68 years for letrozole arm and 3.09 years for tamoxifen arm , showing incremental LYs of 0.59 years in patients receiving letrozole .
	manualset3
152098	6	409945	7	NULL	NULL	0	NULL	incremental LYs	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The expected overall life-years ( LYs ) obtained were 3.68 years for letrozole arm and 3.09 years for tamoxifen arm , showing incremental LYs of 0.59 years in patients receiving letrozole .
	manualset3
152100	7	409945	7	NULL	NULL	0	NULL	 0.59 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The expected overall life-years ( LYs ) obtained were 3.68 years for letrozole arm and 3.09 years for tamoxifen arm , showing incremental LYs of 0.59 years in patients receiving letrozole .
	manualset3
152102	8	409945	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The expected overall life-years ( LYs ) obtained were 3.68 years for letrozole arm and 3.09 years for tamoxifen arm , showing incremental LYs of 0.59 years in patients receiving letrozole .
	manualset3
152104	9	409945	7	NULL	NULL	0	NULL	letrozole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The expected overall life-years ( LYs ) obtained were 3.68 years for letrozole arm and 3.09 years for tamoxifen arm , showing incremental LYs of 0.59 years in patients receiving letrozole .
	manualset3
152112	1	409946	7	NULL	NULL	0	NULL	experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The experience of the Bakulev Institute of Cardiovascular Surgery is shown in illustration of the main organizational measures which allow the number of reconstructive operations in the cardinal branches of angiosurgery to be increased twofold .
	manualset3
152113	2	409946	7	NULL	NULL	0	NULL	Bakulev Institute of Cardiovascular Surgery 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The experience of the Bakulev Institute of Cardiovascular Surgery is shown in illustration of the main organizational measures which allow the number of reconstructive operations in the cardinal branches of angiosurgery to be increased twofold .
	manualset3
152114	3	409946	7	NULL	NULL	0	NULL	illustration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The experience of the Bakulev Institute of Cardiovascular Surgery is shown in illustration of the main organizational measures which allow the number of reconstructive operations in the cardinal branches of angiosurgery to be increased twofold .
	manualset3
152125	4	409946	7	NULL	NULL	NULL	NULL	main organizational measures	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The experience of the Bakulev Institute of Cardiovascular Surgery is shown in illustration of the main organizational measures which allow the number of reconstructive operations in the cardinal branches of angiosurgery to be increased twofold .
	manualset3
152127	5	409946	7	NULL	NULL	0	NULL	number of reconstructive operations 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The experience of the Bakulev Institute of Cardiovascular Surgery is shown in illustration of the main organizational measures which allow the number of reconstructive operations in the cardinal branches of angiosurgery to be increased twofold .
	manualset3
152133	6	409946	7	NULL	NULL	0	NULL	cardinal branches	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The experience of the Bakulev Institute of Cardiovascular Surgery is shown in illustration of the main organizational measures which allow the number of reconstructive operations in the cardinal branches of angiosurgery to be increased twofold .
	manualset3
152135	7	409946	7	NULL	NULL	0	NULL	angiosurgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The experience of the Bakulev Institute of Cardiovascular Surgery is shown in illustration of the main organizational measures which allow the number of reconstructive operations in the cardinal branches of angiosurgery to be increased twofold .
	manualset3
152153	1	409947	7	NULL	NULL	0	NULL	Clinical-statistical investigation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical-statistical investigation of the relation between presumed oral focal infection and antistreptolysin titers ) .
	manualset3
152159	2	409947	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical-statistical investigation of the relation between presumed oral focal infection and antistreptolysin titers ) .
	manualset3
152162	3	409947	7	NULL	NULL	0	NULL	presumed oral focal infection	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical-statistical investigation of the relation between presumed oral focal infection and antistreptolysin titers ) .
	manualset3
152163	4	409947	7	NULL	NULL	0	NULL	antistreptolysin titers	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical-statistical investigation of the relation between presumed oral focal infection and antistreptolysin titers ) .
	manualset3
152178	1	409948	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A study of their amino acid sequences points to an , as yet obscure , interaction between C-terminal f-Met and N-terminal aromatic Phe .
	manualset3
152184	2	409948	7	NULL	NULL	0	NULL	amino acid sequences points	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A study of their amino acid sequences points to an , as yet obscure , interaction between C-terminal f-Met and N-terminal aromatic Phe .
	manualset3
152188	4	409948	7	NULL	NULL	NULL	NULL	C-terminal f-Met	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A study of their amino acid sequences points to an , as yet obscure , interaction between C-terminal f-Met and N-terminal aromatic Phe .
	manualset3
152189	5	409948	7	NULL	NULL	NULL	NULL	N-terminal aromatic Phe	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A study of their amino acid sequences points to an , as yet obscure , interaction between C-terminal f-Met and N-terminal aromatic Phe .
	manualset3
152649	3	409948	7	NULL	NULL	0	NULL	interaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A study of their amino acid sequences points to an , as yet obscure , interaction between C-terminal f-Met and N-terminal aromatic Phe .
	manualset3
152190	1	409949	7	NULL	NULL	0	NULL	experiment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The experiment was performed with a two-phase solvent system composed of methyl tert.-butyl ether-tetrahydrofuran-distilled water ( 2 : 2 : 3 , v/v ) where triethylamine ( 10 mM ) was added to the upper organic stationary phase as a retainer and hydrochloric acid ( 10 mM ) to the aqueous mobile phase as an eluter .
	manualset3
152191	2	409949	7	NULL	NULL	0	NULL	two-phase solvent system	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The experiment was performed with a two-phase solvent system composed of methyl tert.-butyl ether-tetrahydrofuran-distilled water ( 2 : 2 : 3 , v/v ) where triethylamine ( 10 mM ) was added to the upper organic stationary phase as a retainer and hydrochloric acid ( 10 mM ) to the aqueous mobile phase as an eluter .
	manualset3
152192	3	409949	7	NULL	NULL	0	NULL	methyl tert.-butyl ether-tetrahydrofuran-distilled water ( 2 : 2 : 3 , v/v )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The experiment was performed with a two-phase solvent system composed of methyl tert.-butyl ether-tetrahydrofuran-distilled water ( 2 : 2 : 3 , v/v ) where triethylamine ( 10 mM ) was added to the upper organic stationary phase as a retainer and hydrochloric acid ( 10 mM ) to the aqueous mobile phase as an eluter .
	manualset3
152193	4	409949	7	NULL	NULL	0	NULL	triethylamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The experiment was performed with a two-phase solvent system composed of methyl tert.-butyl ether-tetrahydrofuran-distilled water ( 2 : 2 : 3 , v/v ) where triethylamine ( 10 mM ) was added to the upper organic stationary phase as a retainer and hydrochloric acid ( 10 mM ) to the aqueous mobile phase as an eluter .
	manualset3
152194	5	409949	7	NULL	NULL	0	NULL	upper organic stationary phase	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The experiment was performed with a two-phase solvent system composed of methyl tert.-butyl ether-tetrahydrofuran-distilled water ( 2 : 2 : 3 , v/v ) where triethylamine ( 10 mM ) was added to the upper organic stationary phase as a retainer and hydrochloric acid ( 10 mM ) to the aqueous mobile phase as an eluter .
	manualset3
152195	6	409949	7	NULL	NULL	NULL	NULL	retainer	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The experiment was performed with a two-phase solvent system composed of methyl tert.-butyl ether-tetrahydrofuran-distilled water ( 2 : 2 : 3 , v/v ) where triethylamine ( 10 mM ) was added to the upper organic stationary phase as a retainer and hydrochloric acid ( 10 mM ) to the aqueous mobile phase as an eluter .
	manualset3
152196	7	409949	7	NULL	NULL	0	NULL	hydrochloric acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The experiment was performed with a two-phase solvent system composed of methyl tert.-butyl ether-tetrahydrofuran-distilled water ( 2 : 2 : 3 , v/v ) where triethylamine ( 10 mM ) was added to the upper organic stationary phase as a retainer and hydrochloric acid ( 10 mM ) to the aqueous mobile phase as an eluter .
	manualset3
152197	8	409949	7	NULL	NULL	0	NULL	aqueous mobile phase	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The experiment was performed with a two-phase solvent system composed of methyl tert.-butyl ether-tetrahydrofuran-distilled water ( 2 : 2 : 3 , v/v ) where triethylamine ( 10 mM ) was added to the upper organic stationary phase as a retainer and hydrochloric acid ( 10 mM ) to the aqueous mobile phase as an eluter .
	manualset3
152198	9	409949	7	NULL	NULL	0	NULL	eluter	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The experiment was performed with a two-phase solvent system composed of methyl tert.-butyl ether-tetrahydrofuran-distilled water ( 2 : 2 : 3 , v/v ) where triethylamine ( 10 mM ) was added to the upper organic stationary phase as a retainer and hydrochloric acid ( 10 mM ) to the aqueous mobile phase as an eluter .
	manualset3
152199	1	409950	7	NULL	NULL	0	NULL	experimental animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental animals belonging to the Sprague-Dawley-derived strain of our laboratory were kept under standard conditions for food , illumination and temperature .
	manualset3
152200	2	409950	7	NULL	NULL	0	NULL	Sprague-Dawley-derived strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental animals belonging to the Sprague-Dawley-derived strain of our laboratory were kept under standard conditions for food , illumination and temperature .
	manualset3
152201	4	409950	7	NULL	NULL	NULL	NULL	standard conditions	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The experimental animals belonging to the Sprague-Dawley-derived strain of our laboratory were kept under standard conditions for food , illumination and temperature .
	manualset3
152202	5	409950	7	NULL	NULL	NULL	NULL	food	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The experimental animals belonging to the Sprague-Dawley-derived strain of our laboratory were kept under standard conditions for food , illumination and temperature .
	manualset3
152203	6	409950	7	NULL	NULL	NULL	NULL	illumination	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The experimental animals belonging to the Sprague-Dawley-derived strain of our laboratory were kept under standard conditions for food , illumination and temperature .
	manualset3
152204	7	409950	7	NULL	NULL	NULL	NULL	temperature	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The experimental animals belonging to the Sprague-Dawley-derived strain of our laboratory were kept under standard conditions for food , illumination and temperature .
	manualset3
152205	3	409950	7	NULL	NULL	0	NULL	laboratory	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental animals belonging to the Sprague-Dawley-derived strain of our laboratory were kept under standard conditions for food , illumination and temperature .
	manualset3
152206	1	409951	7	NULL	NULL	0	NULL	experimental constraints	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental constraints that transepithelial potential difference is small and that the fractional apical resistance is greater than 85 % mandate that more than 75 % of luminal Na + entry be electrically silent .
	manualset3
152207	2	409951	7	NULL	NULL	0	NULL	 transepithelial potential difference 	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental constraints that transepithelial potential difference is small and that the fractional apical resistance is greater than 85 % mandate that more than 75 % of luminal Na + entry be electrically silent .
	manualset3
152209	3	409951	7	NULL	NULL	NULL	NULL	fractional apical resistance	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The experimental constraints that transepithelial potential difference is small and that the fractional apical resistance is greater than 85 % mandate that more than 75 % of luminal Na + entry be electrically silent .
	manualset3
152210	4	409951	7	NULL	NULL	NULL	NULL	85 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The experimental constraints that transepithelial potential difference is small and that the fractional apical resistance is greater than 85 % mandate that more than 75 % of luminal Na + entry be electrically silent .
	manualset3
152211	5	409951	7	NULL	NULL	NULL	NULL	75 % 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The experimental constraints that transepithelial potential difference is small and that the fractional apical resistance is greater than 85 % mandate that more than 75 % of luminal Na + entry be electrically silent .
	manualset3
152212	6	409951	7	NULL	NULL	NULL	NULL	luminal Na + entry 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The experimental constraints that transepithelial potential difference is small and that the fractional apical resistance is greater than 85 % mandate that more than 75 % of luminal Na + entry be electrically silent .
	manualset3
152214	1	409952	7	NULL	NULL	0	NULL	experimental data	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental data of ammonium exchange by natural Bigadi clinoptilolite was evaluated using nonlinear regression analysis .
	manualset3
152215	2	409952	7	NULL	NULL	0	NULL	ammonium exchange	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental data of ammonium exchange by natural Bigadi clinoptilolite was evaluated using nonlinear regression analysis .
	manualset3
152216	3	409952	7	NULL	NULL	0	NULL	 natural Bigadi clinoptilolite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental data of ammonium exchange by natural Bigadi clinoptilolite was evaluated using nonlinear regression analysis .
	manualset3
152217	4	409952	7	NULL	NULL	0	NULL	nonlinear regression analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental data of ammonium exchange by natural Bigadi clinoptilolite was evaluated using nonlinear regression analysis .
	manualset3
152218	1	409953	7	NULL	NULL	NULL	NULL	experimental design methodology	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The experimental design methodology was first applied to the chemical oxidation process in order to determine the values of temperature , ferrous ion concentration and hydrogen peroxide concentration that maximize dissolved organic carbon ( DOC ) and color removals and increase the effluent 's biodegradability .
	manualset3
152220	2	409953	7	NULL	NULL	NULL	NULL	chemical oxidation process	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The experimental design methodology was first applied to the chemical oxidation process in order to determine the values of temperature , ferrous ion concentration and hydrogen peroxide concentration that maximize dissolved organic carbon ( DOC ) and color removals and increase the effluent 's biodegradability .
	manualset3
152221	3	409953	7	NULL	NULL	NULL	NULL	temperature	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The experimental design methodology was first applied to the chemical oxidation process in order to determine the values of temperature , ferrous ion concentration and hydrogen peroxide concentration that maximize dissolved organic carbon ( DOC ) and color removals and increase the effluent 's biodegradability .
	manualset3
152222	4	409953	7	NULL	NULL	NULL	NULL	ferrous ion concentration	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The experimental design methodology was first applied to the chemical oxidation process in order to determine the values of temperature , ferrous ion concentration and hydrogen peroxide concentration that maximize dissolved organic carbon ( DOC ) and color removals and increase the effluent 's biodegradability .
	manualset3
152223	5	409953	7	NULL	NULL	NULL	NULL	hydrogen peroxide concentration	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The experimental design methodology was first applied to the chemical oxidation process in order to determine the values of temperature , ferrous ion concentration and hydrogen peroxide concentration that maximize dissolved organic carbon ( DOC ) and color removals and increase the effluent 's biodegradability .
	manualset3
152224	6	409953	7	NULL	NULL	NULL	NULL	dissolved organic carbon ( DOC )	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The experimental design methodology was first applied to the chemical oxidation process in order to determine the values of temperature , ferrous ion concentration and hydrogen peroxide concentration that maximize dissolved organic carbon ( DOC ) and color removals and increase the effluent 's biodegradability .
	manualset3
152225	7	409953	7	NULL	NULL	NULL	NULL	color removals	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The experimental design methodology was first applied to the chemical oxidation process in order to determine the values of temperature , ferrous ion concentration and hydrogen peroxide concentration that maximize dissolved organic carbon ( DOC ) and color removals and increase the effluent 's biodegradability .
	manualset3
152226	8	409953	7	NULL	NULL	NULL	NULL	effluent 's biodegradability	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The experimental design methodology was first applied to the chemical oxidation process in order to determine the values of temperature , ferrous ion concentration and hydrogen peroxide concentration that maximize dissolved organic carbon ( DOC ) and color removals and increase the effluent 's biodegradability .
	manualset3
152227	1	409954	7	NULL	NULL	0	NULL	experimental part	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental part of the study employs CDI with short high-voltage pulses , while the theoretical part of the study is based on numerical simulations of MREIT .
	manualset3
152228	2	409954	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental part of the study employs CDI with short high-voltage pulses , while the theoretical part of the study is based on numerical simulations of MREIT .
	manualset3
152229	3	409954	7	NULL	NULL	0	NULL	 CDI	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental part of the study employs CDI with short high-voltage pulses , while the theoretical part of the study is based on numerical simulations of MREIT .
	manualset3
152230	4	409954	7	NULL	NULL	0	NULL	short high-voltage pulses	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental part of the study employs CDI with short high-voltage pulses , while the theoretical part of the study is based on numerical simulations of MREIT .
	manualset3
152231	5	409954	7	NULL	NULL	0	NULL	theoretical part of the study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental part of the study employs CDI with short high-voltage pulses , while the theoretical part of the study is based on numerical simulations of MREIT .
	manualset3
152232	6	409954	7	NULL	NULL	0	NULL	 numerical simulations of MREIT	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental part of the study employs CDI with short high-voltage pulses , while the theoretical part of the study is based on numerical simulations of MREIT .
	manualset3
152664	1	409955	7	NULL	NULL	0	NULL	experimental procedures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental procedures for viral nanoindentation experiments are described here in detail , focusing on surface preparation , AFM imaging and nanoindentation , and the subsequent data analysis of the force-distance curves .
	manualset3
152665	2	409955	7	NULL	NULL	NULL	NULL	viral nanoindentation experiments	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The experimental procedures for viral nanoindentation experiments are described here in detail , focusing on surface preparation , AFM imaging and nanoindentation , and the subsequent data analysis of the force-distance curves .
	manualset3
152666	3	409955	7	NULL	NULL	NULL	NULL	surface preparation	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The experimental procedures for viral nanoindentation experiments are described here in detail , focusing on surface preparation , AFM imaging and nanoindentation , and the subsequent data analysis of the force-distance curves .
	manualset3
152667	4	409955	7	NULL	NULL	0	NULL	AFM imaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental procedures for viral nanoindentation experiments are described here in detail , focusing on surface preparation , AFM imaging and nanoindentation , and the subsequent data analysis of the force-distance curves .
	manualset3
152668	5	409955	7	NULL	NULL	0	NULL	nanoindentation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental procedures for viral nanoindentation experiments are described here in detail , focusing on surface preparation , AFM imaging and nanoindentation , and the subsequent data analysis of the force-distance curves .
	manualset3
152669	6	409955	7	NULL	NULL	0	NULL	subsequent data analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental procedures for viral nanoindentation experiments are described here in detail , focusing on surface preparation , AFM imaging and nanoindentation , and the subsequent data analysis of the force-distance curves .
	manualset3
152670	7	409955	7	NULL	NULL	0	NULL	 force-distance curves	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental procedures for viral nanoindentation experiments are described here in detail , focusing on surface preparation , AFM imaging and nanoindentation , and the subsequent data analysis of the force-distance curves .
	manualset3
152671	1	409956	7	NULL	NULL	NULL	NULL	experimental results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The experimental results indicate that increasing the number of screws enhances the cup stability in the case of ideal screwing ( i.e. , with no eccentricity ) .
	manualset3
152673	2	409956	7	NULL	NULL	NULL	NULL	cup stability	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The experimental results indicate that increasing the number of screws enhances the cup stability in the case of ideal screwing ( i.e. , with no eccentricity ) .
	manualset3
152676	3	409956	7	NULL	NULL	NULL	NULL	ideal screwing	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The experimental results indicate that increasing the number of screws enhances the cup stability in the case of ideal screwing ( i.e. , with no eccentricity ) .
	manualset3
157162	4	409956	7	NULL	NULL	0	NULL	number of screws	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental results indicate that increasing the number of screws enhances the cup stability in the case of ideal screwing ( i.e. , with no eccentricity ) .
	manualset3
157163	5	409956	7	NULL	NULL	0	NULL	 no eccentricity	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental results indicate that increasing the number of screws enhances the cup stability in the case of ideal screwing ( i.e. , with no eccentricity ) .
	manualset3
152678	1	409957	7	NULL	NULL	0	NULL	experimental results	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental results may provide useful data for the design of pyrolytic processing systems using planktonic microalgae as feedstock .
	manualset3
152679	2	409957	7	NULL	NULL	NULL	NULL	 data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The experimental results may provide useful data for the design of pyrolytic processing systems using planktonic microalgae as feedstock .
	manualset3
152680	3	409957	7	NULL	NULL	0	NULL	design of pyrolytic processing systems	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental results may provide useful data for the design of pyrolytic processing systems using planktonic microalgae as feedstock .
	manualset3
152681	4	409957	7	NULL	NULL	0	NULL	 planktonic microalgae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental results may provide useful data for the design of pyrolytic processing systems using planktonic microalgae as feedstock .
	manualset3
152682	5	409957	7	NULL	NULL	0	NULL	feedstock	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental results may provide useful data for the design of pyrolytic processing systems using planktonic microalgae as feedstock .
	manualset3
152683	1	409958	7	NULL	NULL	0	NULL	experimental results	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental results suggest that increases in Na/Pi cotransporter mRNA and protein may mediate the increase in Na/Pi cotransport activity in OK cells during phosphate depletion .
	manualset3
152684	2	409958	7	NULL	NULL	0	NULL	Na/Pi cotransporter mRNA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental results suggest that increases in Na/Pi cotransporter mRNA and protein may mediate the increase in Na/Pi cotransport activity in OK cells during phosphate depletion .
	manualset3
152685	3	409958	7	NULL	NULL	0	NULL	Na/Pi cotransporter protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental results suggest that increases in Na/Pi cotransporter mRNA and protein may mediate the increase in Na/Pi cotransport activity in OK cells during phosphate depletion .
	manualset3
152686	4	409958	7	NULL	NULL	0	NULL	Na/Pi cotransport activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental results suggest that increases in Na/Pi cotransporter mRNA and protein may mediate the increase in Na/Pi cotransport activity in OK cells during phosphate depletion .
	manualset3
152687	5	409958	7	NULL	NULL	0	NULL	OK cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental results suggest that increases in Na/Pi cotransporter mRNA and protein may mediate the increase in Na/Pi cotransport activity in OK cells during phosphate depletion .
	manualset3
152688	6	409958	7	NULL	NULL	0	NULL	phosphate depletion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental results suggest that increases in Na/Pi cotransporter mRNA and protein may mediate the increase in Na/Pi cotransport activity in OK cells during phosphate depletion .
	manualset3
157165	7	409958	7	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimental results suggest that increases in Na/Pi cotransporter mRNA and protein may mediate the increase in Na/Pi cotransport activity in OK cells during phosphate depletion .
	manualset3
152689	1	409959	7	NULL	NULL	NULL	NULL	experimentally determined orbital interaction energies 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The experimentally determined orbital interaction energies reveal a previously unidentified overlap interaction of the predominantly sulfur HOMO of the bdt ligand with filled orbitals of the Cp ligands , suggesting that direct dithiolene interactions with other ligands bound to the metal could be significant for other metal-dithiolene systems in chemistry and biology .
	manualset3
152691	3	409959	7	NULL	NULL	0	NULL	unidentified overlap interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimentally determined orbital interaction energies reveal a previously unidentified overlap interaction of the predominantly sulfur HOMO of the bdt ligand with filled orbitals of the Cp ligands , suggesting that direct dithiolene interactions with other ligands bound to the metal could be significant for other metal-dithiolene systems in chemistry and biology .
	manualset3
152692	4	409959	7	NULL	NULL	NULL	NULL	sulfur HOMO	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The experimentally determined orbital interaction energies reveal a previously unidentified overlap interaction of the predominantly sulfur HOMO of the bdt ligand with filled orbitals of the Cp ligands , suggesting that direct dithiolene interactions with other ligands bound to the metal could be significant for other metal-dithiolene systems in chemistry and biology .
	manualset3
152693	5	409959	7	NULL	NULL	0	NULL	bdt ligand	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimentally determined orbital interaction energies reveal a previously unidentified overlap interaction of the predominantly sulfur HOMO of the bdt ligand with filled orbitals of the Cp ligands , suggesting that direct dithiolene interactions with other ligands bound to the metal could be significant for other metal-dithiolene systems in chemistry and biology .
	manualset3
152694	6	409959	7	NULL	NULL	0	NULL	filled orbitals	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimentally determined orbital interaction energies reveal a previously unidentified overlap interaction of the predominantly sulfur HOMO of the bdt ligand with filled orbitals of the Cp ligands , suggesting that direct dithiolene interactions with other ligands bound to the metal could be significant for other metal-dithiolene systems in chemistry and biology .
	manualset3
152695	7	409959	7	NULL	NULL	0	NULL	Cp ligands	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimentally determined orbital interaction energies reveal a previously unidentified overlap interaction of the predominantly sulfur HOMO of the bdt ligand with filled orbitals of the Cp ligands , suggesting that direct dithiolene interactions with other ligands bound to the metal could be significant for other metal-dithiolene systems in chemistry and biology .
	manualset3
152696	8	409959	7	NULL	NULL	0	NULL	direct dithiolene interactions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimentally determined orbital interaction energies reveal a previously unidentified overlap interaction of the predominantly sulfur HOMO of the bdt ligand with filled orbitals of the Cp ligands , suggesting that direct dithiolene interactions with other ligands bound to the metal could be significant for other metal-dithiolene systems in chemistry and biology .
	manualset3
152697	9	409959	7	NULL	NULL	0	NULL	ligands	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimentally determined orbital interaction energies reveal a previously unidentified overlap interaction of the predominantly sulfur HOMO of the bdt ligand with filled orbitals of the Cp ligands , suggesting that direct dithiolene interactions with other ligands bound to the metal could be significant for other metal-dithiolene systems in chemistry and biology .
	manualset3
152698	10	409959	7	NULL	NULL	NULL	NULL	metal	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The experimentally determined orbital interaction energies reveal a previously unidentified overlap interaction of the predominantly sulfur HOMO of the bdt ligand with filled orbitals of the Cp ligands , suggesting that direct dithiolene interactions with other ligands bound to the metal could be significant for other metal-dithiolene systems in chemistry and biology .
	manualset3
152699	11	409959	7	NULL	NULL	0	NULL	metal-dithiolene systems	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimentally determined orbital interaction energies reveal a previously unidentified overlap interaction of the predominantly sulfur HOMO of the bdt ligand with filled orbitals of the Cp ligands , suggesting that direct dithiolene interactions with other ligands bound to the metal could be significant for other metal-dithiolene systems in chemistry and biology .
	manualset3
152700	12	409959	7	NULL	NULL	0	NULL	chemistry	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimentally determined orbital interaction energies reveal a previously unidentified overlap interaction of the predominantly sulfur HOMO of the bdt ligand with filled orbitals of the Cp ligands , suggesting that direct dithiolene interactions with other ligands bound to the metal could be significant for other metal-dithiolene systems in chemistry and biology .
	manualset3
152701	13	409959	7	NULL	NULL	0	NULL	biology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The experimentally determined orbital interaction energies reveal a previously unidentified overlap interaction of the predominantly sulfur HOMO of the bdt ligand with filled orbitals of the Cp ligands , suggesting that direct dithiolene interactions with other ligands bound to the metal could be significant for other metal-dithiolene systems in chemistry and biology .
	manualset3
152702	1	409960	7	NULL	NULL	0	NULL	experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The experiments were conducted with suspensions of Escherichia coli and Bacillus thuringiensis cells subjected to the action of heat , toluene , ethanol , and freezing .
	manualset3
152703	2	409960	7	NULL	NULL	0	NULL	suspensions of Escherichia coli 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The experiments were conducted with suspensions of Escherichia coli and Bacillus thuringiensis cells subjected to the action of heat , toluene , ethanol , and freezing .
	manualset3
152704	3	409960	7	NULL	NULL	0	NULL	Bacillus thuringiensis cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The experiments were conducted with suspensions of Escherichia coli and Bacillus thuringiensis cells subjected to the action of heat , toluene , ethanol , and freezing .
	manualset3
152705	4	409960	7	NULL	NULL	0	NULL	action of heat	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The experiments were conducted with suspensions of Escherichia coli and Bacillus thuringiensis cells subjected to the action of heat , toluene , ethanol , and freezing .
	manualset3
152706	5	409960	7	NULL	NULL	0	NULL	toluene 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The experiments were conducted with suspensions of Escherichia coli and Bacillus thuringiensis cells subjected to the action of heat , toluene , ethanol , and freezing .
	manualset3
152707	6	409960	7	NULL	NULL	0	NULL	ethanol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The experiments were conducted with suspensions of Escherichia coli and Bacillus thuringiensis cells subjected to the action of heat , toluene , ethanol , and freezing .
	manualset3
152708	7	409960	7	NULL	NULL	0	NULL	freezing 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The experiments were conducted with suspensions of Escherichia coli and Bacillus thuringiensis cells subjected to the action of heat , toluene , ethanol , and freezing .
	manualset3
152713	1	409961	7	NULL	NULL	0	NULL	experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The experiments with activated carbon sorbent indicated that phenyl groups in activated carbon structure and aldrin molecules exhibited competitive behavior on reaction with OH * radicals .
	manualset3
152820	2	409961	7	NULL	NULL	0	NULL	activated carbon sorbent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The experiments with activated carbon sorbent indicated that phenyl groups in activated carbon structure and aldrin molecules exhibited competitive behavior on reaction with OH * radicals .
	manualset3
152821	3	409961	7	NULL	NULL	0	NULL	phenyl groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The experiments with activated carbon sorbent indicated that phenyl groups in activated carbon structure and aldrin molecules exhibited competitive behavior on reaction with OH * radicals .
	manualset3
152825	4	409961	7	NULL	NULL	0	NULL	activated carbon structure	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The experiments with activated carbon sorbent indicated that phenyl groups in activated carbon structure and aldrin molecules exhibited competitive behavior on reaction with OH * radicals .
	manualset3
152826	5	409961	7	NULL	NULL	0	NULL	aldrin molecules	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The experiments with activated carbon sorbent indicated that phenyl groups in activated carbon structure and aldrin molecules exhibited competitive behavior on reaction with OH * radicals .
	manualset3
152827	6	409961	7	NULL	NULL	0	NULL	competitive behavior 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The experiments with activated carbon sorbent indicated that phenyl groups in activated carbon structure and aldrin molecules exhibited competitive behavior on reaction with OH * radicals .
	manualset3
152828	7	409961	7	NULL	NULL	0	NULL	 reaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The experiments with activated carbon sorbent indicated that phenyl groups in activated carbon structure and aldrin molecules exhibited competitive behavior on reaction with OH * radicals .
	manualset3
152829	8	409961	7	NULL	NULL	0	NULL	OH * radicals	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The experiments with activated carbon sorbent indicated that phenyl groups in activated carbon structure and aldrin molecules exhibited competitive behavior on reaction with OH * radicals .
	manualset3
152831	1	409962	7	NULL	NULL	NULL	NULL	expert system	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expert system thus seems to perform well .
	manualset3
152832	2	409962	7	NULL	NULL	0	NULL	perform	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The expert system thus seems to perform well .
	manualset3
152833	3	409962	7	NULL	NULL	0	NULL	well	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The expert system thus seems to perform well .
	manualset3
152835	1	409963	7	NULL	NULL	0	NULL	 exploitation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The exploitation of such naturally produced antagonists holds tremendous potential for extension of shelf-life and improvement of safety of a variety of foods .
	manualset3
152836	2	409963	7	NULL	NULL	0	NULL	naturally produced antagonists	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The exploitation of such naturally produced antagonists holds tremendous potential for extension of shelf-life and improvement of safety of a variety of foods .
	manualset3
152837	3	409963	7	NULL	NULL	0	NULL	tremendous potential 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The exploitation of such naturally produced antagonists holds tremendous potential for extension of shelf-life and improvement of safety of a variety of foods .
	manualset3
152838	4	409963	7	NULL	NULL	0	NULL	extension of shelf-life	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The exploitation of such naturally produced antagonists holds tremendous potential for extension of shelf-life and improvement of safety of a variety of foods .
	manualset3
152839	5	409963	7	NULL	NULL	0	NULL	improvement of safety	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The exploitation of such naturally produced antagonists holds tremendous potential for extension of shelf-life and improvement of safety of a variety of foods .
	manualset3
152841	6	409963	7	NULL	NULL	0	NULL	variety of foods	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The exploitation of such naturally produced antagonists holds tremendous potential for extension of shelf-life and improvement of safety of a variety of foods .
	manualset3
152842	1	409964	7	NULL	NULL	0	NULL	expression levels	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression levels of other connexins expressed in heart ( Cx37 , Cx43 and Cx45 ) were the same in Cx40 - / - and Cx40 + / + mice .
	manualset3
152843	2	409964	7	NULL	NULL	0	NULL	connexins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression levels of other connexins expressed in heart ( Cx37 , Cx43 and Cx45 ) were the same in Cx40 - / - and Cx40 + / + mice .
	manualset3
152844	3	409964	7	NULL	NULL	NULL	NULL	heart	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression levels of other connexins expressed in heart ( Cx37 , Cx43 and Cx45 ) were the same in Cx40 - / - and Cx40 + / + mice .
	manualset3
152846	4	409964	7	NULL	NULL	0	NULL	Cx37	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression levels of other connexins expressed in heart ( Cx37 , Cx43 and Cx45 ) were the same in Cx40 - / - and Cx40 + / + mice .
	manualset3
152848	5	409964	7	NULL	NULL	0	NULL	Cx43	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression levels of other connexins expressed in heart ( Cx37 , Cx43 and Cx45 ) were the same in Cx40 - / - and Cx40 + / + mice .
	manualset3
152850	6	409964	7	NULL	NULL	0	NULL	Cx45	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression levels of other connexins expressed in heart ( Cx37 , Cx43 and Cx45 ) were the same in Cx40 - / - and Cx40 + / + mice .
	manualset3
152852	7	409964	7	NULL	NULL	0	NULL	Cx40 - / - mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression levels of other connexins expressed in heart ( Cx37 , Cx43 and Cx45 ) were the same in Cx40 - / - and Cx40 + / + mice .
	manualset3
152853	8	409964	7	NULL	NULL	0	NULL	Cx40 + / + mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression levels of other connexins expressed in heart ( Cx37 , Cx43 and Cx45 ) were the same in Cx40 - / - and Cx40 + / + mice .
	manualset3
152855	1	409965	7	NULL	NULL	0	NULL	expression	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of BMPR-IB and BMPR-II mRNA was up-regulated by HGF , as shown by both conventional PCR and quantitative PCR .
	manualset3
152859	2	409965	7	NULL	NULL	0	NULL	BMPR-IB mRNA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of BMPR-IB and BMPR-II mRNA was up-regulated by HGF , as shown by both conventional PCR and quantitative PCR .
	manualset3
152860	3	409965	7	NULL	NULL	0	NULL	BMPR-II mRNA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of BMPR-IB and BMPR-II mRNA was up-regulated by HGF , as shown by both conventional PCR and quantitative PCR .
	manualset3
152861	4	409965	7	NULL	NULL	NULL	NULL	up-regulated 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of BMPR-IB and BMPR-II mRNA was up-regulated by HGF , as shown by both conventional PCR and quantitative PCR .
	manualset3
152865	5	409965	7	NULL	NULL	0	NULL	HGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of BMPR-IB and BMPR-II mRNA was up-regulated by HGF , as shown by both conventional PCR and quantitative PCR .
	manualset3
152867	6	409965	7	NULL	NULL	0	NULL	conventional PCR 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of BMPR-IB and BMPR-II mRNA was up-regulated by HGF , as shown by both conventional PCR and quantitative PCR .
	manualset3
152868	7	409965	7	NULL	NULL	0	NULL	quantitative PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of BMPR-IB and BMPR-II mRNA was up-regulated by HGF , as shown by both conventional PCR and quantitative PCR .
	manualset3
152871	1	409966	7	NULL	NULL	NULL	NULL	expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of CA150 , measured immunohistochemically , was markedly increased in human HD brain tissue compared with normal age-matched human brain tissue , and CA150 showed aggregate formation with partial colocalization to ubiquitin-positive aggregates .
	manualset3
152872	2	409966	7	NULL	NULL	0	NULL	CA150 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of CA150 , measured immunohistochemically , was markedly increased in human HD brain tissue compared with normal age-matched human brain tissue , and CA150 showed aggregate formation with partial colocalization to ubiquitin-positive aggregates .
	manualset3
152880	3	409966	7	NULL	NULL	NULL	NULL	human HD brain tissue	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of CA150 , measured immunohistochemically , was markedly increased in human HD brain tissue compared with normal age-matched human brain tissue , and CA150 showed aggregate formation with partial colocalization to ubiquitin-positive aggregates .
	manualset3
152886	4	409966	7	NULL	NULL	NULL	NULL	human brain tissue	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of CA150 , measured immunohistochemically , was markedly increased in human HD brain tissue compared with normal age-matched human brain tissue , and CA150 showed aggregate formation with partial colocalization to ubiquitin-positive aggregates .
	manualset3
152889	5	409966	7	NULL	NULL	NULL	NULL	CA150	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of CA150 , measured immunohistochemically , was markedly increased in human HD brain tissue compared with normal age-matched human brain tissue , and CA150 showed aggregate formation with partial colocalization to ubiquitin-positive aggregates .
	manualset3
152891	6	409966	7	NULL	NULL	NULL	NULL	aggregate formation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of CA150 , measured immunohistochemically , was markedly increased in human HD brain tissue compared with normal age-matched human brain tissue , and CA150 showed aggregate formation with partial colocalization to ubiquitin-positive aggregates .
	manualset3
152892	7	409966	7	NULL	NULL	NULL	NULL	partial colocalization	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of CA150 , measured immunohistochemically , was markedly increased in human HD brain tissue compared with normal age-matched human brain tissue , and CA150 showed aggregate formation with partial colocalization to ubiquitin-positive aggregates .
	manualset3
152893	8	409966	7	NULL	NULL	NULL	NULL	ubiquitin-positive aggregates	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of CA150 , measured immunohistochemically , was markedly increased in human HD brain tissue compared with normal age-matched human brain tissue , and CA150 showed aggregate formation with partial colocalization to ubiquitin-positive aggregates .
	manualset3
152894	1	409967	7	NULL	NULL	0	NULL	expression	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of GALT was characterized both in vivo and in vitro during late embryonic and postnatal development of the brain and peripheral nerve of the rat .
	manualset3
152895	2	409967	7	NULL	NULL	0	NULL	GALT 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of GALT was characterized both in vivo and in vitro during late embryonic and postnatal development of the brain and peripheral nerve of the rat .
	manualset3
152898	5	409967	7	NULL	NULL	NULL	NULL	late embryonic development of the brain	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of GALT was characterized both in vivo and in vitro during late embryonic and postnatal development of the brain and peripheral nerve of the rat .
	manualset3
152899	6	409967	7	NULL	NULL	0	NULL	postnatal development of the brain 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of GALT was characterized both in vivo and in vitro during late embryonic and postnatal development of the brain and peripheral nerve of the rat .
	manualset3
152900	7	409967	7	NULL	NULL	NULL	NULL	peripheral nerve	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of GALT was characterized both in vivo and in vitro during late embryonic and postnatal development of the brain and peripheral nerve of the rat .
	manualset3
152901	8	409967	7	NULL	NULL	0	NULL	rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of GALT was characterized both in vivo and in vitro during late embryonic and postnatal development of the brain and peripheral nerve of the rat .
	manualset3
152902	1	409968	7	NULL	NULL	NULL	NULL	expression 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of GTK also correlates with a markedly increased content of FAK , phosphorylation of the adaptor protein Shb , and an association between these two proteins .
	manualset3
152903	2	409968	7	NULL	NULL	0	NULL	GTK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of GTK also correlates with a markedly increased content of FAK , phosphorylation of the adaptor protein Shb , and an association between these two proteins .
	manualset3
152904	3	409968	7	NULL	NULL	NULL	NULL	 increased content	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of GTK also correlates with a markedly increased content of FAK , phosphorylation of the adaptor protein Shb , and an association between these two proteins .
	manualset3
152905	4	409968	7	NULL	NULL	0	NULL	FAK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of GTK also correlates with a markedly increased content of FAK , phosphorylation of the adaptor protein Shb , and an association between these two proteins .
	manualset3
152906	5	409968	7	NULL	NULL	0	NULL	phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of GTK also correlates with a markedly increased content of FAK , phosphorylation of the adaptor protein Shb , and an association between these two proteins .
	manualset3
152907	6	409968	7	NULL	NULL	0	NULL	adaptor protein Shb	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of GTK also correlates with a markedly increased content of FAK , phosphorylation of the adaptor protein Shb , and an association between these two proteins .
	manualset3
152908	7	409968	7	NULL	NULL	0	NULL	association 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of GTK also correlates with a markedly increased content of FAK , phosphorylation of the adaptor protein Shb , and an association between these two proteins .
	manualset3
152909	8	409968	7	NULL	NULL	0	NULL	two proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of GTK also correlates with a markedly increased content of FAK , phosphorylation of the adaptor protein Shb , and an association between these two proteins .
	manualset3
152910	1	409969	7	NULL	NULL	NULL	NULL	expression 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of IL-17A , IL-10 , IL-6 , and TGF - mRNAs were higher in the bleomycin group than in the normal group .
	manualset3
152911	2	409969	7	NULL	NULL	0	NULL	IL-17A mRNA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of IL-17A , IL-10 , IL-6 , and TGF - mRNAs were higher in the bleomycin group than in the normal group .
	manualset3
152912	3	409969	7	NULL	NULL	0	NULL	IL-10 mRNA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of IL-17A , IL-10 , IL-6 , and TGF - mRNAs were higher in the bleomycin group than in the normal group .
	manualset3
152913	4	409969	7	NULL	NULL	0	NULL	IL-6 mRNA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of IL-17A , IL-10 , IL-6 , and TGF - mRNAs were higher in the bleomycin group than in the normal group .
	manualset3
152914	5	409969	7	NULL	NULL	0	NULL	TGF - mRNA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of IL-17A , IL-10 , IL-6 , and TGF - mRNAs were higher in the bleomycin group than in the normal group .
	manualset3
152915	6	409969	7	NULL	NULL	0	NULL	 bleomycin group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of IL-17A , IL-10 , IL-6 , and TGF - mRNAs were higher in the bleomycin group than in the normal group .
	manualset3
152916	7	409969	7	NULL	NULL	0	NULL	normal group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of IL-17A , IL-10 , IL-6 , and TGF - mRNAs were higher in the bleomycin group than in the normal group .
	manualset3
152917	1	409970	7	NULL	NULL	NULL	NULL	expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of PSD-95 in the hippocampus might be regulated by fragile X mental retardation protein ( FMRP ) during mice early developmental and adult periods .
	manualset3
152922	2	409970	7	NULL	NULL	0	NULL	PSD-95	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of PSD-95 in the hippocampus might be regulated by fragile X mental retardation protein ( FMRP ) during mice early developmental and adult periods .
	manualset3
152924	3	409970	7	NULL	NULL	0	NULL	hippocampus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of PSD-95 in the hippocampus might be regulated by fragile X mental retardation protein ( FMRP ) during mice early developmental and adult periods .
	manualset3
152927	4	409970	7	NULL	NULL	0	NULL	fragile X mental retardation protein ( FMRP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of PSD-95 in the hippocampus might be regulated by fragile X mental retardation protein ( FMRP ) during mice early developmental and adult periods .
	manualset3
152929	5	409970	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of PSD-95 in the hippocampus might be regulated by fragile X mental retardation protein ( FMRP ) during mice early developmental and adult periods .
	manualset3
152931	6	409970	7	NULL	NULL	0	NULL	early developmental period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of PSD-95 in the hippocampus might be regulated by fragile X mental retardation protein ( FMRP ) during mice early developmental and adult periods .
	manualset3
152932	7	409970	7	NULL	NULL	0	NULL	adult period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of PSD-95 in the hippocampus might be regulated by fragile X mental retardation protein ( FMRP ) during mice early developmental and adult periods .
	manualset3
152935	1	409971	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A study was carried out in the in-vitro rat phrenic nerve hemidiaphragm preparation to find a fast and strong working antagonist of non-depolarizing muscle relaxants .
	manualset3
152936	2	409971	7	NULL	NULL	NULL	NULL	in-vitro preparation	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A study was carried out in the in-vitro rat phrenic nerve hemidiaphragm preparation to find a fast and strong working antagonist of non-depolarizing muscle relaxants .
	manualset3
152937	3	409971	7	NULL	NULL	0	NULL	rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A study was carried out in the in-vitro rat phrenic nerve hemidiaphragm preparation to find a fast and strong working antagonist of non-depolarizing muscle relaxants .
	manualset3
152938	4	409971	7	NULL	NULL	NULL	NULL	phrenic nerve hemidiaphragm 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A study was carried out in the in-vitro rat phrenic nerve hemidiaphragm preparation to find a fast and strong working antagonist of non-depolarizing muscle relaxants .
	manualset3
152942	5	409971	7	NULL	NULL	NULL	NULL	strong working antagonist	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A study was carried out in the in-vitro rat phrenic nerve hemidiaphragm preparation to find a fast and strong working antagonist of non-depolarizing muscle relaxants .
	manualset3
152946	6	409971	7	NULL	NULL	NULL	NULL	non-depolarizing muscle relaxants	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A study was carried out in the in-vitro rat phrenic nerve hemidiaphragm preparation to find a fast and strong working antagonist of non-depolarizing muscle relaxants .
	manualset3
153019	1	409972	7	NULL	NULL	NULL	NULL	 expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of PdtK , the outer membrane receptor involved in PDTC transport , was also reduced in response to added zinc whereas other iron-regulated outer membrane proteins were not .
	manualset3
153022	2	409972	7	NULL	NULL	0	NULL	PdtK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of PdtK , the outer membrane receptor involved in PDTC transport , was also reduced in response to added zinc whereas other iron-regulated outer membrane proteins were not .
	manualset3
153025	3	409972	7	NULL	NULL	0	NULL	 outer membrane receptor	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of PdtK , the outer membrane receptor involved in PDTC transport , was also reduced in response to added zinc whereas other iron-regulated outer membrane proteins were not .
	manualset3
153026	4	409972	7	NULL	NULL	NULL	NULL	PDTC transport	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of PdtK , the outer membrane receptor involved in PDTC transport , was also reduced in response to added zinc whereas other iron-regulated outer membrane proteins were not .
	manualset3
153028	5	409972	7	NULL	NULL	0	NULL	 zinc	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of PdtK , the outer membrane receptor involved in PDTC transport , was also reduced in response to added zinc whereas other iron-regulated outer membrane proteins were not .
	manualset3
153029	6	409972	7	NULL	NULL	0	NULL	 iron-regulated outer membrane proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of PdtK , the outer membrane receptor involved in PDTC transport , was also reduced in response to added zinc whereas other iron-regulated outer membrane proteins were not .
	manualset3
153030	1	409973	7	NULL	NULL	NULL	NULL	expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of Rt6-1 and Rt6-2 mRNAs in lymphoid tissues suggests that these ARTs may regulate immune system functions .
	manualset3
153031	2	409973	7	NULL	NULL	0	NULL	Rt6-1 mRNA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of Rt6-1 and Rt6-2 mRNAs in lymphoid tissues suggests that these ARTs may regulate immune system functions .
	manualset3
153032	3	409973	7	NULL	NULL	0	NULL	Rt6-2 mRNA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of Rt6-1 and Rt6-2 mRNAs in lymphoid tissues suggests that these ARTs may regulate immune system functions .
	manualset3
153033	4	409973	7	NULL	NULL	0	NULL	lymphoid tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of Rt6-1 and Rt6-2 mRNAs in lymphoid tissues suggests that these ARTs may regulate immune system functions .
	manualset3
153034	5	409973	7	NULL	NULL	NULL	NULL	ARTs	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of Rt6-1 and Rt6-2 mRNAs in lymphoid tissues suggests that these ARTs may regulate immune system functions .
	manualset3
153038	6	409973	7	NULL	NULL	0	NULL	immune system functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of Rt6-1 and Rt6-2 mRNAs in lymphoid tissues suggests that these ARTs may regulate immune system functions .
	manualset3
153045	1	409974	7	NULL	NULL	NULL	NULL	 expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of TNFSF13 mRNA in DLPFC correlated negatively with tissue pH , but decreasing pH in cultured cells did not cause increased TNFSF13 mRNA nor did exogenous TNFSF13 decrease pH. .
	manualset3
153046	2	409974	7	NULL	NULL	0	NULL	TNFSF13 mRNA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of TNFSF13 mRNA in DLPFC correlated negatively with tissue pH , but decreasing pH in cultured cells did not cause increased TNFSF13 mRNA nor did exogenous TNFSF13 decrease pH. .
	manualset3
153047	3	409974	7	NULL	NULL	0	NULL	DLPFC	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of TNFSF13 mRNA in DLPFC correlated negatively with tissue pH , but decreasing pH in cultured cells did not cause increased TNFSF13 mRNA nor did exogenous TNFSF13 decrease pH. .
	manualset3
153048	4	409974	7	NULL	NULL	0	NULL	tissue pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of TNFSF13 mRNA in DLPFC correlated negatively with tissue pH , but decreasing pH in cultured cells did not cause increased TNFSF13 mRNA nor did exogenous TNFSF13 decrease pH. .
	manualset3
153049	5	409974	7	NULL	NULL	0	NULL	decreasing pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of TNFSF13 mRNA in DLPFC correlated negatively with tissue pH , but decreasing pH in cultured cells did not cause increased TNFSF13 mRNA nor did exogenous TNFSF13 decrease pH. .
	manualset3
153050	6	409974	7	NULL	NULL	0	NULL	cultured cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of TNFSF13 mRNA in DLPFC correlated negatively with tissue pH , but decreasing pH in cultured cells did not cause increased TNFSF13 mRNA nor did exogenous TNFSF13 decrease pH. .
	manualset3
153051	7	409974	7	NULL	NULL	0	NULL	 increased TNFSF13 mRNA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of TNFSF13 mRNA in DLPFC correlated negatively with tissue pH , but decreasing pH in cultured cells did not cause increased TNFSF13 mRNA nor did exogenous TNFSF13 decrease pH. .
	manualset3
153052	8	409974	7	NULL	NULL	0	NULL	exogenous TNFSF13	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of TNFSF13 mRNA in DLPFC correlated negatively with tissue pH , but decreasing pH in cultured cells did not cause increased TNFSF13 mRNA nor did exogenous TNFSF13 decrease pH. .
	manualset3
153054	10	409974	7	NULL	NULL	0	NULL	pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of TNFSF13 mRNA in DLPFC correlated negatively with tissue pH , but decreasing pH in cultured cells did not cause increased TNFSF13 mRNA nor did exogenous TNFSF13 decrease pH. .
	manualset3
153058	1	409975	7	NULL	NULL	NULL	NULL	expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of an 11-transcript subset related to the degree of proteinuria , and this 11-mRNA subset was also sufficient to distinguish biopsies of subjects with IgAN from control biopsies .
	manualset3
153060	2	409975	7	NULL	NULL	NULL	NULL	11-transcript subset	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of an 11-transcript subset related to the degree of proteinuria , and this 11-mRNA subset was also sufficient to distinguish biopsies of subjects with IgAN from control biopsies .
	manualset3
153062	3	409975	7	NULL	NULL	NULL	NULL	degree of proteinuria	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of an 11-transcript subset related to the degree of proteinuria , and this 11-mRNA subset was also sufficient to distinguish biopsies of subjects with IgAN from control biopsies .
	manualset3
153063	4	409975	7	NULL	NULL	NULL	NULL	11-mRNA subset	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of an 11-transcript subset related to the degree of proteinuria , and this 11-mRNA subset was also sufficient to distinguish biopsies of subjects with IgAN from control biopsies .
	manualset3
153064	5	409975	7	NULL	NULL	NULL	NULL	biopsies	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of an 11-transcript subset related to the degree of proteinuria , and this 11-mRNA subset was also sufficient to distinguish biopsies of subjects with IgAN from control biopsies .
	manualset3
153065	6	409975	7	NULL	NULL	NULL	NULL	subjects	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of an 11-transcript subset related to the degree of proteinuria , and this 11-mRNA subset was also sufficient to distinguish biopsies of subjects with IgAN from control biopsies .
	manualset3
153071	7	409975	7	NULL	NULL	NULL	NULL	 IgAN	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of an 11-transcript subset related to the degree of proteinuria , and this 11-mRNA subset was also sufficient to distinguish biopsies of subjects with IgAN from control biopsies .
	manualset3
153073	8	409975	7	NULL	NULL	NULL	NULL	 control biopsies 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of an 11-transcript subset related to the degree of proteinuria , and this 11-mRNA subset was also sufficient to distinguish biopsies of subjects with IgAN from control biopsies .
	manualset3
153084	1	409976	7	NULL	NULL	NULL	NULL	expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of beta-tubulin and troponin increased significantly in the transfected group as compared with the non-transfected group .
	manualset3
153085	2	409976	7	NULL	NULL	0	NULL	beta-tubulin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of beta-tubulin and troponin increased significantly in the transfected group as compared with the non-transfected group .
	manualset3
153086	3	409976	7	NULL	NULL	0	NULL	troponin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of beta-tubulin and troponin increased significantly in the transfected group as compared with the non-transfected group .
	manualset3
153087	4	409976	7	NULL	NULL	0	NULL	transfected group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of beta-tubulin and troponin increased significantly in the transfected group as compared with the non-transfected group .
	manualset3
153088	5	409976	7	NULL	NULL	0	NULL	non-transfected group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of beta-tubulin and troponin increased significantly in the transfected group as compared with the non-transfected group .
	manualset3
153093	1	409977	7	NULL	NULL	NULL	NULL	expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of cartilage-characteristic genes decreased with the progression of bone maturation .
	manualset3
153094	2	409977	7	NULL	NULL	0	NULL	 cartilage-characteristic genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of cartilage-characteristic genes decreased with the progression of bone maturation .
	manualset3
153095	3	409977	7	NULL	NULL	0	NULL	progression	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of cartilage-characteristic genes decreased with the progression of bone maturation .
	manualset3
153096	4	409977	7	NULL	NULL	0	NULL	bone maturation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of cartilage-characteristic genes decreased with the progression of bone maturation .
	manualset3
153099	1	409978	7	NULL	NULL	NULL	NULL	expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of floral organ identity genes in contrasting water lily cultivars .
	manualset3
153101	2	409978	7	NULL	NULL	0	NULL	floral organ identity genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of floral organ identity genes in contrasting water lily cultivars .
	manualset3
153102	3	409978	7	NULL	NULL	0	NULL	water lily cultivars 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of floral organ identity genes in contrasting water lily cultivars .
	manualset3
153104	1	409979	7	NULL	NULL	NULL	NULL	expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of galectin-3 has been studied in a rat model of acute mesangial proliferative glomerulonephritis in which a single injection of anti-Thy1 .1 antibodies leads to destruction of mesangial cells expressing a Thy1 .1 epitope on their surface .
	manualset3
153108	2	409979	7	NULL	NULL	0	NULL	galectin-3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of galectin-3 has been studied in a rat model of acute mesangial proliferative glomerulonephritis in which a single injection of anti-Thy1 .1 antibodies leads to destruction of mesangial cells expressing a Thy1 .1 epitope on their surface .
	manualset3
153111	3	409979	7	NULL	NULL	0	NULL	 rat model 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of galectin-3 has been studied in a rat model of acute mesangial proliferative glomerulonephritis in which a single injection of anti-Thy1 .1 antibodies leads to destruction of mesangial cells expressing a Thy1 .1 epitope on their surface .
	manualset3
153114	4	409979	7	NULL	NULL	0	NULL	acute mesangial proliferative glomerulonephritis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of galectin-3 has been studied in a rat model of acute mesangial proliferative glomerulonephritis in which a single injection of anti-Thy1 .1 antibodies leads to destruction of mesangial cells expressing a Thy1 .1 epitope on their surface .
	manualset3
153116	5	409979	7	NULL	NULL	0	NULL	single injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of galectin-3 has been studied in a rat model of acute mesangial proliferative glomerulonephritis in which a single injection of anti-Thy1 .1 antibodies leads to destruction of mesangial cells expressing a Thy1 .1 epitope on their surface .
	manualset3
153119	6	409979	7	NULL	NULL	0	NULL	anti-Thy1 .1 antibodies	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of galectin-3 has been studied in a rat model of acute mesangial proliferative glomerulonephritis in which a single injection of anti-Thy1 .1 antibodies leads to destruction of mesangial cells expressing a Thy1 .1 epitope on their surface .
	manualset3
153120	7	409979	7	NULL	NULL	0	NULL	destruction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of galectin-3 has been studied in a rat model of acute mesangial proliferative glomerulonephritis in which a single injection of anti-Thy1 .1 antibodies leads to destruction of mesangial cells expressing a Thy1 .1 epitope on their surface .
	manualset3
153121	8	409979	7	NULL	NULL	0	NULL	mesangial cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of galectin-3 has been studied in a rat model of acute mesangial proliferative glomerulonephritis in which a single injection of anti-Thy1 .1 antibodies leads to destruction of mesangial cells expressing a Thy1 .1 epitope on their surface .
	manualset3
153123	9	409979	7	NULL	NULL	0	NULL	Thy1 .1 epitope 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of galectin-3 has been studied in a rat model of acute mesangial proliferative glomerulonephritis in which a single injection of anti-Thy1 .1 antibodies leads to destruction of mesangial cells expressing a Thy1 .1 epitope on their surface .
	manualset3
153125	10	409979	7	NULL	NULL	0	NULL	surface	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of galectin-3 has been studied in a rat model of acute mesangial proliferative glomerulonephritis in which a single injection of anti-Thy1 .1 antibodies leads to destruction of mesangial cells expressing a Thy1 .1 epitope on their surface .
	manualset3
153129	1	409980	7	NULL	NULL	NULL	NULL	expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of gp200 , which appears to have tyrosine kinase activity and is immunologically related to the EGF receptor in tumor cells , suggests its possible involvement in cell growth .
	manualset3
153130	2	409980	7	NULL	NULL	0	NULL	gp200	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of gp200 , which appears to have tyrosine kinase activity and is immunologically related to the EGF receptor in tumor cells , suggests its possible involvement in cell growth .
	manualset3
153131	3	409980	7	NULL	NULL	0	NULL	 tyrosine kinase activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of gp200 , which appears to have tyrosine kinase activity and is immunologically related to the EGF receptor in tumor cells , suggests its possible involvement in cell growth .
	manualset3
153132	4	409980	7	NULL	NULL	0	NULL	 EGF receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of gp200 , which appears to have tyrosine kinase activity and is immunologically related to the EGF receptor in tumor cells , suggests its possible involvement in cell growth .
	manualset3
153133	5	409980	7	NULL	NULL	NULL	NULL	tumor cells	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of gp200 , which appears to have tyrosine kinase activity and is immunologically related to the EGF receptor in tumor cells , suggests its possible involvement in cell growth .
	manualset3
153134	6	409980	7	NULL	NULL	0	NULL	cell growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of gp200 , which appears to have tyrosine kinase activity and is immunologically related to the EGF receptor in tumor cells , suggests its possible involvement in cell growth .
	manualset3
153858	1	409981	7	NULL	NULL	NULL	NULL	expression 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of mRNAs encoding 13 GABAA receptor subunits ( alpha 1-6 , beta 1-3 , gamma 1-3 , and delta ) in embryonic , postnatal , and adult rat spinal cord and dorsal root ganglia ( DRG ) cells were studied by in situ hybridization and reverse transcription-polymerase chain reaction ( RT-PCR ) analysis .
	manualset3
153859	2	409981	7	NULL	NULL	NULL	NULL	13 GABAA receptor subunits ( alpha 1-6 , beta 1-3 , gamma 1-3 , and delta )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression of mRNAs encoding 13 GABAA receptor subunits ( alpha 1-6 , beta 1-3 , gamma 1-3 , and delta ) in embryonic , postnatal , and adult rat spinal cord and dorsal root ganglia ( DRG ) cells were studied by in situ hybridization and reverse transcription-polymerase chain reaction ( RT-PCR ) analysis .
	manualset3
153860	3	409981	7	NULL	NULL	0	NULL	embryonic rat spinal cord	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of mRNAs encoding 13 GABAA receptor subunits ( alpha 1-6 , beta 1-3 , gamma 1-3 , and delta ) in embryonic , postnatal , and adult rat spinal cord and dorsal root ganglia ( DRG ) cells were studied by in situ hybridization and reverse transcription-polymerase chain reaction ( RT-PCR ) analysis .
	manualset3
153861	4	409981	7	NULL	NULL	0	NULL	postnatal rat spinal cord	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of mRNAs encoding 13 GABAA receptor subunits ( alpha 1-6 , beta 1-3 , gamma 1-3 , and delta ) in embryonic , postnatal , and adult rat spinal cord and dorsal root ganglia ( DRG ) cells were studied by in situ hybridization and reverse transcription-polymerase chain reaction ( RT-PCR ) analysis .
	manualset3
153862	5	409981	7	NULL	NULL	0	NULL	adult rat spinal cord	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of mRNAs encoding 13 GABAA receptor subunits ( alpha 1-6 , beta 1-3 , gamma 1-3 , and delta ) in embryonic , postnatal , and adult rat spinal cord and dorsal root ganglia ( DRG ) cells were studied by in situ hybridization and reverse transcription-polymerase chain reaction ( RT-PCR ) analysis .
	manualset3
153863	6	409981	7	NULL	NULL	0	NULL	dorsal root ganglia ( DRG ) cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of mRNAs encoding 13 GABAA receptor subunits ( alpha 1-6 , beta 1-3 , gamma 1-3 , and delta ) in embryonic , postnatal , and adult rat spinal cord and dorsal root ganglia ( DRG ) cells were studied by in situ hybridization and reverse transcription-polymerase chain reaction ( RT-PCR ) analysis .
	manualset3
153864	7	409981	7	NULL	NULL	0	NULL	in situ hybridization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of mRNAs encoding 13 GABAA receptor subunits ( alpha 1-6 , beta 1-3 , gamma 1-3 , and delta ) in embryonic , postnatal , and adult rat spinal cord and dorsal root ganglia ( DRG ) cells were studied by in situ hybridization and reverse transcription-polymerase chain reaction ( RT-PCR ) analysis .
	manualset3
153865	8	409981	7	NULL	NULL	0	NULL	reverse transcription-polymerase chain reaction ( RT-PCR ) analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of mRNAs encoding 13 GABAA receptor subunits ( alpha 1-6 , beta 1-3 , gamma 1-3 , and delta ) in embryonic , postnatal , and adult rat spinal cord and dorsal root ganglia ( DRG ) cells were studied by in situ hybridization and reverse transcription-polymerase chain reaction ( RT-PCR ) analysis .
	manualset3
153866	9	409981	7	NULL	NULL	0	NULL	mRNAs	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of mRNAs encoding 13 GABAA receptor subunits ( alpha 1-6 , beta 1-3 , gamma 1-3 , and delta ) in embryonic , postnatal , and adult rat spinal cord and dorsal root ganglia ( DRG ) cells were studied by in situ hybridization and reverse transcription-polymerase chain reaction ( RT-PCR ) analysis .
	manualset3
153867	1	409982	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A study was undertaken to evaluate the ion-beam texturing of aluminum oxide as a means of providing a surface which will produce a biological prosthetic attachment .
	manualset3
153868	2	409982	7	NULL	NULL	0	NULL	ion-beam texturing	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A study was undertaken to evaluate the ion-beam texturing of aluminum oxide as a means of providing a surface which will produce a biological prosthetic attachment .
	manualset3
153869	3	409982	7	NULL	NULL	NULL	NULL	aluminum oxide	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A study was undertaken to evaluate the ion-beam texturing of aluminum oxide as a means of providing a surface which will produce a biological prosthetic attachment .
	manualset3
153870	4	409982	7	NULL	NULL	NULL	NULL	surface	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A study was undertaken to evaluate the ion-beam texturing of aluminum oxide as a means of providing a surface which will produce a biological prosthetic attachment .
	manualset3
153871	5	409982	7	NULL	NULL	NULL	NULL	biological prosthetic attachment	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A study was undertaken to evaluate the ion-beam texturing of aluminum oxide as a means of providing a surface which will produce a biological prosthetic attachment .
	manualset3
157164	6	409982	7	NULL	NULL	0	NULL	evaluate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A study was undertaken to evaluate the ion-beam texturing of aluminum oxide as a means of providing a surface which will produce a biological prosthetic attachment .
	manualset3
153872	1	409983	7	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of the genes for somatostatin ( SRIF ) and brain-derived neurotrophic factor ( BDNF ) was investigated in the central nervous system ( CNS ) of the macaque monkey ( Macaca fuscata fuscata ) .
	manualset3
153873	2	409983	7	NULL	NULL	0	NULL	genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of the genes for somatostatin ( SRIF ) and brain-derived neurotrophic factor ( BDNF ) was investigated in the central nervous system ( CNS ) of the macaque monkey ( Macaca fuscata fuscata ) .
	manualset3
153874	3	409983	7	NULL	NULL	0	NULL	 somatostatin ( SRIF ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of the genes for somatostatin ( SRIF ) and brain-derived neurotrophic factor ( BDNF ) was investigated in the central nervous system ( CNS ) of the macaque monkey ( Macaca fuscata fuscata ) .
	manualset3
153875	4	409983	7	NULL	NULL	0	NULL	brain-derived neurotrophic factor ( BDNF )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of the genes for somatostatin ( SRIF ) and brain-derived neurotrophic factor ( BDNF ) was investigated in the central nervous system ( CNS ) of the macaque monkey ( Macaca fuscata fuscata ) .
	manualset3
153876	5	409983	7	NULL	NULL	0	NULL	 central nervous system ( CNS )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of the genes for somatostatin ( SRIF ) and brain-derived neurotrophic factor ( BDNF ) was investigated in the central nervous system ( CNS ) of the macaque monkey ( Macaca fuscata fuscata ) .
	manualset3
153877	6	409983	7	NULL	NULL	0	NULL	macaque monkey ( Macaca fuscata fuscata )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression of the genes for somatostatin ( SRIF ) and brain-derived neurotrophic factor ( BDNF ) was investigated in the central nervous system ( CNS ) of the macaque monkey ( Macaca fuscata fuscata ) .
	manualset3
153878	1	409984	7	NULL	NULL	NULL	NULL	expression profile	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression profile of TLR9 mRNA and CpG ODNs immunostimulatory actions in the teleost gilthead seabream points to a major role of lymphocytes .
	manualset3
153879	2	409984	7	NULL	NULL	NULL	NULL	TLR9 mRNA	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expression profile of TLR9 mRNA and CpG ODNs immunostimulatory actions in the teleost gilthead seabream points to a major role of lymphocytes .
	manualset3
153880	3	409984	7	NULL	NULL	0	NULL	CpG ODNs immunostimulatory actions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression profile of TLR9 mRNA and CpG ODNs immunostimulatory actions in the teleost gilthead seabream points to a major role of lymphocytes .
	manualset3
153881	4	409984	7	NULL	NULL	0	NULL	teleost gilthead seabream	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression profile of TLR9 mRNA and CpG ODNs immunostimulatory actions in the teleost gilthead seabream points to a major role of lymphocytes .
	manualset3
153882	5	409984	7	NULL	NULL	0	NULL	lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The expression profile of TLR9 mRNA and CpG ODNs immunostimulatory actions in the teleost gilthead seabream points to a major role of lymphocytes .
	manualset3
153883	1	409985	7	NULL	NULL	NULL	NULL	extent of angiogenesis 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The extent of angiogenesis correlates with the increased invasion and metastasis in a variety of human neoplasms .
	manualset3
153884	2	409985	7	NULL	NULL	NULL	NULL	increased invasion	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The extent of angiogenesis correlates with the increased invasion and metastasis in a variety of human neoplasms .
	manualset3
153885	3	409985	7	NULL	NULL	NULL	NULL	metastasis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The extent of angiogenesis correlates with the increased invasion and metastasis in a variety of human neoplasms .
	manualset3
153886	4	409985	7	NULL	NULL	0	NULL	 human neoplasms	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The extent of angiogenesis correlates with the increased invasion and metastasis in a variety of human neoplasms .
	manualset3
153887	1	409986	7	NULL	NULL	0	NULL	extent of incision	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The extent of incision of the two substrates upon addition of UvrC ( 70 % for the psoralen adduct and 20 % for the thymine dimer ) was proportional to the extent of formation of the UvrA-UvrB-DNA ( i.e. UvrB-DNA ) complex , indicating that substrate discrimination occurs at the preincision step .
	manualset3
153888	2	409986	7	NULL	NULL	0	NULL	two substrates	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The extent of incision of the two substrates upon addition of UvrC ( 70 % for the psoralen adduct and 20 % for the thymine dimer ) was proportional to the extent of formation of the UvrA-UvrB-DNA ( i.e. UvrB-DNA ) complex , indicating that substrate discrimination occurs at the preincision step .
	manualset3
153889	3	409986	7	NULL	NULL	0	NULL	UvrC	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The extent of incision of the two substrates upon addition of UvrC ( 70 % for the psoralen adduct and 20 % for the thymine dimer ) was proportional to the extent of formation of the UvrA-UvrB-DNA ( i.e. UvrB-DNA ) complex , indicating that substrate discrimination occurs at the preincision step .
	manualset3
153890	4	409986	7	NULL	NULL	0	NULL	70 % for the psoralen adduct	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The extent of incision of the two substrates upon addition of UvrC ( 70 % for the psoralen adduct and 20 % for the thymine dimer ) was proportional to the extent of formation of the UvrA-UvrB-DNA ( i.e. UvrB-DNA ) complex , indicating that substrate discrimination occurs at the preincision step .
	manualset3
153891	5	409986	7	NULL	NULL	0	NULL	20 % for the thymine dimer	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The extent of incision of the two substrates upon addition of UvrC ( 70 % for the psoralen adduct and 20 % for the thymine dimer ) was proportional to the extent of formation of the UvrA-UvrB-DNA ( i.e. UvrB-DNA ) complex , indicating that substrate discrimination occurs at the preincision step .
	manualset3
153892	6	409986	7	NULL	NULL	NULL	NULL	UvrA-UvrB-DNA complex	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The extent of incision of the two substrates upon addition of UvrC ( 70 % for the psoralen adduct and 20 % for the thymine dimer ) was proportional to the extent of formation of the UvrA-UvrB-DNA ( i.e. UvrB-DNA ) complex , indicating that substrate discrimination occurs at the preincision step .
	manualset3
153893	7	409986	7	NULL	NULL	0	NULL	substrate discrimination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The extent of incision of the two substrates upon addition of UvrC ( 70 % for the psoralen adduct and 20 % for the thymine dimer ) was proportional to the extent of formation of the UvrA-UvrB-DNA ( i.e. UvrB-DNA ) complex , indicating that substrate discrimination occurs at the preincision step .
	manualset3
153894	8	409986	7	NULL	NULL	0	NULL	preincision step	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The extent of incision of the two substrates upon addition of UvrC ( 70 % for the psoralen adduct and 20 % for the thymine dimer ) was proportional to the extent of formation of the UvrA-UvrB-DNA ( i.e. UvrB-DNA ) complex , indicating that substrate discrimination occurs at the preincision step .
	manualset3
154439	9	409986	7	NULL	NULL	NULL	NULL	 UvrB-DNA  complex	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The extent of incision of the two substrates upon addition of UvrC ( 70 % for the psoralen adduct and 20 % for the thymine dimer ) was proportional to the extent of formation of the UvrA-UvrB-DNA ( i.e. UvrB-DNA ) complex , indicating that substrate discrimination occurs at the preincision step .
	manualset3
153895	1	409987	7	NULL	NULL	0	NULL	extent	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The extent of pre-admission risk factor management was also determined .
	manualset3
153896	2	409987	7	NULL	NULL	0	NULL	pre-admission risk factor management	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The extent of pre-admission risk factor management was also determined .
	manualset3
153900	1	409988	7	NULL	NULL	0	NULL	extent 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The extent to which changes in dietary habits , both during pregnancy and in later life , may act to contribute to the current explosion in childhood and adult obesity remains a scientific and public health challenge to us all .
	manualset3
153901	2	409988	7	NULL	NULL	NULL	NULL	 dietary habits	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The extent to which changes in dietary habits , both during pregnancy and in later life , may act to contribute to the current explosion in childhood and adult obesity remains a scientific and public health challenge to us all .
	manualset3
153902	3	409988	7	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The extent to which changes in dietary habits , both during pregnancy and in later life , may act to contribute to the current explosion in childhood and adult obesity remains a scientific and public health challenge to us all .
	manualset3
153903	4	409988	7	NULL	NULL	0	NULL	later life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The extent to which changes in dietary habits , both during pregnancy and in later life , may act to contribute to the current explosion in childhood and adult obesity remains a scientific and public health challenge to us all .
	manualset3
153904	5	409988	7	NULL	NULL	0	NULL	current explosion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The extent to which changes in dietary habits , both during pregnancy and in later life , may act to contribute to the current explosion in childhood and adult obesity remains a scientific and public health challenge to us all .
	manualset3
153909	6	409988	7	NULL	NULL	0	NULL	childhood	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The extent to which changes in dietary habits , both during pregnancy and in later life , may act to contribute to the current explosion in childhood and adult obesity remains a scientific and public health challenge to us all .
	manualset3
153912	7	409988	7	NULL	NULL	0	NULL	adult obesity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The extent to which changes in dietary habits , both during pregnancy and in later life , may act to contribute to the current explosion in childhood and adult obesity remains a scientific and public health challenge to us all .
	manualset3
153916	8	409988	7	NULL	NULL	0	NULL	public health challenge	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The extent to which changes in dietary habits , both during pregnancy and in later life , may act to contribute to the current explosion in childhood and adult obesity remains a scientific and public health challenge to us all .
	manualset3
153917	1	409989	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A study with recombinant polypeptides of the human acetylcholine receptor alpha-subunit .
	manualset3
153918	2	409989	7	NULL	NULL	0	NULL	recombinant polypeptides	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A study with recombinant polypeptides of the human acetylcholine receptor alpha-subunit .
	manualset3
153919	3	409989	7	NULL	NULL	0	NULL	human acetylcholine receptor alpha-subunit	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A study with recombinant polypeptides of the human acetylcholine receptor alpha-subunit .
	manualset3
153920	1	409990	7	NULL	NULL	0	NULL	extracellular Ca ( 2 + ) - sensing receptor ( CaR ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The extracellular Ca ( 2 + ) - sensing receptor ( CaR ) , a G protein-coupled receptor responsible for maintenance of calcium homeostasis , is implicated in regulation of skeletal metabolism .
	manualset3
153922	2	409990	7	NULL	NULL	0	NULL	G protein-coupled receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The extracellular Ca ( 2 + ) - sensing receptor ( CaR ) , a G protein-coupled receptor responsible for maintenance of calcium homeostasis , is implicated in regulation of skeletal metabolism .
	manualset3
153923	3	409990	7	NULL	NULL	0	NULL	calcium homeostasis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The extracellular Ca ( 2 + ) - sensing receptor ( CaR ) , a G protein-coupled receptor responsible for maintenance of calcium homeostasis , is implicated in regulation of skeletal metabolism .
	manualset3
153924	5	409990	7	NULL	NULL	NULL	NULL	skeletal metabolism	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The extracellular Ca ( 2 + ) - sensing receptor ( CaR ) , a G protein-coupled receptor responsible for maintenance of calcium homeostasis , is implicated in regulation of skeletal metabolism .
	manualset3
154778	4	409990	7	NULL	NULL	0	NULL	regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The extracellular Ca ( 2 + ) - sensing receptor ( CaR ) , a G protein-coupled receptor responsible for maintenance of calcium homeostasis , is implicated in regulation of skeletal metabolism .
	manualset3
153936	1	409991	7	NULL	NULL	0	NULL	extracellular domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The extracellular domain of BPAG2 has a loop structure in the carboxy terminal flexible tail in vivo .
	manualset3
153937	2	409991	7	NULL	NULL	0	NULL	BPAG2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The extracellular domain of BPAG2 has a loop structure in the carboxy terminal flexible tail in vivo .
	manualset3
153944	3	409991	7	NULL	NULL	0	NULL	loop structure	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The extracellular domain of BPAG2 has a loop structure in the carboxy terminal flexible tail in vivo .
	manualset3
153950	4	409991	7	NULL	NULL	0	NULL	carboxy terminal flexible tail 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The extracellular domain of BPAG2 has a loop structure in the carboxy terminal flexible tail in vivo .
	manualset3
153952	1	409992	7	NULL	NULL	NULL	NULL	extracellular matrix ( ECM )	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The extracellular matrix ( ECM ) is a key component in the remodeling process , and increases in collagen occur in the infarct area to replace necrotic myocytes and form a scar .
	manualset3
153953	2	409992	7	NULL	NULL	NULL	NULL	remodeling process	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The extracellular matrix ( ECM ) is a key component in the remodeling process , and increases in collagen occur in the infarct area to replace necrotic myocytes and form a scar .
	manualset3
153954	3	409992	7	NULL	NULL	0	NULL	collagen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The extracellular matrix ( ECM ) is a key component in the remodeling process , and increases in collagen occur in the infarct area to replace necrotic myocytes and form a scar .
	manualset3
153955	4	409992	7	NULL	NULL	0	NULL	 infarct area	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The extracellular matrix ( ECM ) is a key component in the remodeling process , and increases in collagen occur in the infarct area to replace necrotic myocytes and form a scar .
	manualset3
153956	5	409992	7	NULL	NULL	0	NULL	necrotic myocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The extracellular matrix ( ECM ) is a key component in the remodeling process , and increases in collagen occur in the infarct area to replace necrotic myocytes and form a scar .
	manualset3
153957	6	409992	7	NULL	NULL	0	NULL	 scar	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The extracellular matrix ( ECM ) is a key component in the remodeling process , and increases in collagen occur in the infarct area to replace necrotic myocytes and form a scar .
	manualset3
153958	1	409993	7	NULL	NULL	0	NULL	extracranial portion	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The extracranial portion of the internal carotid artery was 2.5 mm of diameter .
	manualset3
153959	2	409993	7	NULL	NULL	0	NULL	internal carotid artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The extracranial portion of the internal carotid artery was 2.5 mm of diameter .
	manualset3
153960	3	409993	7	NULL	NULL	0	NULL	2.5 mm of diameter	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The extracranial portion of the internal carotid artery was 2.5 mm of diameter .
	manualset3
153964	1	409994	7	NULL	NULL	0	NULL	extract	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The extract , HexL , DichL , lupeol and betulin were able to inhibit acetic acid-induced writhing .
	manualset3
153965	2	409994	7	NULL	NULL	0	NULL	HexL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The extract , HexL , DichL , lupeol and betulin were able to inhibit acetic acid-induced writhing .
	manualset3
153966	3	409994	7	NULL	NULL	0	NULL	DichL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The extract , HexL , DichL , lupeol and betulin were able to inhibit acetic acid-induced writhing .
	manualset3
153967	4	409994	7	NULL	NULL	0	NULL	lupeol	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The extract , HexL , DichL , lupeol and betulin were able to inhibit acetic acid-induced writhing .
	manualset3
153968	5	409994	7	NULL	NULL	0	NULL	betulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The extract , HexL , DichL , lupeol and betulin were able to inhibit acetic acid-induced writhing .
	manualset3
153969	6	409994	7	NULL	NULL	0	NULL	acetic acid-induced writhing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The extract , HexL , DichL , lupeol and betulin were able to inhibit acetic acid-induced writhing .
	manualset3
153970	1	409995	7	NULL	NULL	0	NULL	extract	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The extract significantly suppressed postprandial hyperglycemia and blood glycated hemoglobin in the db/db mice .
	manualset3
153971	2	409995	7	NULL	NULL	0	NULL	postprandial hyperglycemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The extract significantly suppressed postprandial hyperglycemia and blood glycated hemoglobin in the db/db mice .
	manualset3
153972	3	409995	7	NULL	NULL	NULL	NULL	blood glycated hemoglobin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The extract significantly suppressed postprandial hyperglycemia and blood glycated hemoglobin in the db/db mice .
	manualset3
153973	4	409995	7	NULL	NULL	0	NULL	db/db mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The extract significantly suppressed postprandial hyperglycemia and blood glycated hemoglobin in the db/db mice .
	manualset3
153983	1	409996	7	NULL	NULL	0	NULL	extraction 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The extraction of epidermal growth factor showed no significant difference .
	manualset3
153984	2	409996	7	NULL	NULL	0	NULL	epidermal growth factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The extraction of epidermal growth factor showed no significant difference .
	manualset3
153985	3	409996	7	NULL	NULL	NULL	NULL	no significant difference	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The extraction of epidermal growth factor showed no significant difference .
	manualset3
153986	1	409997	7	NULL	NULL	NULL	NULL	extraction yields	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The extraction yields and purities were found to be directly related to the intensity of the carbonyl vibration at 1713 cm ( -1 ) in the FTIR spectrum of the used BC batch .
	manualset3
153987	2	409997	7	NULL	NULL	NULL	NULL	extraction purities	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The extraction yields and purities were found to be directly related to the intensity of the carbonyl vibration at 1713 cm ( -1 ) in the FTIR spectrum of the used BC batch .
	manualset3
153988	3	409997	7	NULL	NULL	NULL	NULL	intensity of the carbonyl vibration	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The extraction yields and purities were found to be directly related to the intensity of the carbonyl vibration at 1713 cm ( -1 ) in the FTIR spectrum of the used BC batch .
	manualset3
153989	4	409997	7	NULL	NULL	0	NULL	1713 cm ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The extraction yields and purities were found to be directly related to the intensity of the carbonyl vibration at 1713 cm ( -1 ) in the FTIR spectrum of the used BC batch .
	manualset3
153990	5	409997	7	NULL	NULL	0	NULL	FTIR spectrum	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The extraction yields and purities were found to be directly related to the intensity of the carbonyl vibration at 1713 cm ( -1 ) in the FTIR spectrum of the used BC batch .
	manualset3
153991	6	409997	7	NULL	NULL	NULL	NULL	 BC batch	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The extraction yields and purities were found to be directly related to the intensity of the carbonyl vibration at 1713 cm ( -1 ) in the FTIR spectrum of the used BC batch .
	manualset3
153992	1	409998	7	NULL	NULL	0	NULL	extreme mesial	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The extreme mesial and lateral enamel was neither typical of inner nor of outer enamel .
	manualset3
153993	2	409998	7	NULL	NULL	0	NULL	 lateral enamel	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The extreme mesial and lateral enamel was neither typical of inner nor of outer enamel .
	manualset3
153994	3	409998	7	NULL	NULL	0	NULL	inner nor of outer enamel	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The extreme mesial and lateral enamel was neither typical of inner nor of outer enamel .
	manualset3
154011	1	409999	7	NULL	NULL	0	NULL	facets with a coronal plane	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The facets with a coronal plane are resistant to lateral bending and rotational forces , but those with a sagittal plane are unstable resulting in more shearing stress to the intervertebral discs .
	manualset3
154012	2	409999	7	NULL	NULL	NULL	NULL	 lateral bending 	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The facets with a coronal plane are resistant to lateral bending and rotational forces , but those with a sagittal plane are unstable resulting in more shearing stress to the intervertebral discs .
	manualset3
154013	3	409999	7	NULL	NULL	NULL	NULL	rotational forces	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The facets with a coronal plane are resistant to lateral bending and rotational forces , but those with a sagittal plane are unstable resulting in more shearing stress to the intervertebral discs .
	manualset3
154014	4	409999	7	NULL	NULL	0	NULL	sagittal plane	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The facets with a coronal plane are resistant to lateral bending and rotational forces , but those with a sagittal plane are unstable resulting in more shearing stress to the intervertebral discs .
	manualset3
154016	6	409999	7	NULL	NULL	0	NULL	shearing stress	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The facets with a coronal plane are resistant to lateral bending and rotational forces , but those with a sagittal plane are unstable resulting in more shearing stress to the intervertebral discs .
	manualset3
154017	7	409999	7	NULL	NULL	0	NULL	 intervertebral discs 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The facets with a coronal plane are resistant to lateral bending and rotational forces , but those with a sagittal plane are unstable resulting in more shearing stress to the intervertebral discs .
	manualset3
154018	1	410000	7	NULL	NULL	0	NULL	facial nucleus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The facial nucleus of the guinea pig was divided cytoarchitectonically into the dorsolateral , lateral , intermediate , medio-intermediate , medial , and ventromedial divisions ; the ventromedial division was further divided into the major , dorsal and lateral parts .
	manualset3
154019	2	410000	7	NULL	NULL	NULL	NULL	guinea pig	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The facial nucleus of the guinea pig was divided cytoarchitectonically into the dorsolateral , lateral , intermediate , medio-intermediate , medial , and ventromedial divisions ; the ventromedial division was further divided into the major , dorsal and lateral parts .
	manualset3
154020	3	410000	7	NULL	NULL	0	NULL	dorsolateral divisions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The facial nucleus of the guinea pig was divided cytoarchitectonically into the dorsolateral , lateral , intermediate , medio-intermediate , medial , and ventromedial divisions ; the ventromedial division was further divided into the major , dorsal and lateral parts .
	manualset3
154021	4	410000	7	NULL	NULL	0	NULL	lateral divisions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The facial nucleus of the guinea pig was divided cytoarchitectonically into the dorsolateral , lateral , intermediate , medio-intermediate , medial , and ventromedial divisions ; the ventromedial division was further divided into the major , dorsal and lateral parts .
	manualset3
154022	5	410000	7	NULL	NULL	0	NULL	 intermediate divisions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The facial nucleus of the guinea pig was divided cytoarchitectonically into the dorsolateral , lateral , intermediate , medio-intermediate , medial , and ventromedial divisions ; the ventromedial division was further divided into the major , dorsal and lateral parts .
	manualset3
154023	6	410000	7	NULL	NULL	0	NULL	medio-intermediate divisions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The facial nucleus of the guinea pig was divided cytoarchitectonically into the dorsolateral , lateral , intermediate , medio-intermediate , medial , and ventromedial divisions ; the ventromedial division was further divided into the major , dorsal and lateral parts .
	manualset3
154024	7	410000	7	NULL	NULL	0	NULL	medial divisions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The facial nucleus of the guinea pig was divided cytoarchitectonically into the dorsolateral , lateral , intermediate , medio-intermediate , medial , and ventromedial divisions ; the ventromedial division was further divided into the major , dorsal and lateral parts .
	manualset3
154025	8	410000	7	NULL	NULL	0	NULL	ventromedial divisions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The facial nucleus of the guinea pig was divided cytoarchitectonically into the dorsolateral , lateral , intermediate , medio-intermediate , medial , and ventromedial divisions ; the ventromedial division was further divided into the major , dorsal and lateral parts .
	manualset3
154026	9	410000	7	NULL	NULL	0	NULL	major parts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The facial nucleus of the guinea pig was divided cytoarchitectonically into the dorsolateral , lateral , intermediate , medio-intermediate , medial , and ventromedial divisions ; the ventromedial division was further divided into the major , dorsal and lateral parts .
	manualset3
154027	10	410000	7	NULL	NULL	0	NULL	dorsal parts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The facial nucleus of the guinea pig was divided cytoarchitectonically into the dorsolateral , lateral , intermediate , medio-intermediate , medial , and ventromedial divisions ; the ventromedial division was further divided into the major , dorsal and lateral parts .
	manualset3
154028	11	410000	7	NULL	NULL	0	NULL	 lateral parts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The facial nucleus of the guinea pig was divided cytoarchitectonically into the dorsolateral , lateral , intermediate , medio-intermediate , medial , and ventromedial divisions ; the ventromedial division was further divided into the major , dorsal and lateral parts .
	manualset3
154029	1	410001	7	NULL	NULL	0	NULL	long-term preservation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact of long-term preservation of the physicochemical properties of DNA molecules in aqueous solutions in complexes with methylresorcinol , hexylresorcinol , and tyrosol , the chemical analogs of microbial autoregulators ( d1 factors ) from the group of alkylhydroxybenzenes ( AOB ) , was established .
	manualset3
154030	2	410001	7	NULL	NULL	0	NULL	 physicochemical properties	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact of long-term preservation of the physicochemical properties of DNA molecules in aqueous solutions in complexes with methylresorcinol , hexylresorcinol , and tyrosol , the chemical analogs of microbial autoregulators ( d1 factors ) from the group of alkylhydroxybenzenes ( AOB ) , was established .
	manualset3
154031	3	410001	7	NULL	NULL	0	NULL	DNA molecules	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact of long-term preservation of the physicochemical properties of DNA molecules in aqueous solutions in complexes with methylresorcinol , hexylresorcinol , and tyrosol , the chemical analogs of microbial autoregulators ( d1 factors ) from the group of alkylhydroxybenzenes ( AOB ) , was established .
	manualset3
154032	4	410001	7	NULL	NULL	0	NULL	aqueous solutions	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact of long-term preservation of the physicochemical properties of DNA molecules in aqueous solutions in complexes with methylresorcinol , hexylresorcinol , and tyrosol , the chemical analogs of microbial autoregulators ( d1 factors ) from the group of alkylhydroxybenzenes ( AOB ) , was established .
	manualset3
154033	5	410001	7	NULL	NULL	0	NULL	methylresorcinol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact of long-term preservation of the physicochemical properties of DNA molecules in aqueous solutions in complexes with methylresorcinol , hexylresorcinol , and tyrosol , the chemical analogs of microbial autoregulators ( d1 factors ) from the group of alkylhydroxybenzenes ( AOB ) , was established .
	manualset3
154034	6	410001	7	NULL	NULL	0	NULL	hexylresorcinol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact of long-term preservation of the physicochemical properties of DNA molecules in aqueous solutions in complexes with methylresorcinol , hexylresorcinol , and tyrosol , the chemical analogs of microbial autoregulators ( d1 factors ) from the group of alkylhydroxybenzenes ( AOB ) , was established .
	manualset3
154035	7	410001	7	NULL	NULL	0	NULL	tyrosol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact of long-term preservation of the physicochemical properties of DNA molecules in aqueous solutions in complexes with methylresorcinol , hexylresorcinol , and tyrosol , the chemical analogs of microbial autoregulators ( d1 factors ) from the group of alkylhydroxybenzenes ( AOB ) , was established .
	manualset3
154037	8	410001	7	NULL	NULL	0	NULL	 microbial autoregulators ( d1 factors )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact of long-term preservation of the physicochemical properties of DNA molecules in aqueous solutions in complexes with methylresorcinol , hexylresorcinol , and tyrosol , the chemical analogs of microbial autoregulators ( d1 factors ) from the group of alkylhydroxybenzenes ( AOB ) , was established .
	manualset3
154038	9	410001	7	NULL	NULL	0	NULL	alkylhydroxybenzenes ( AOB )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact of long-term preservation of the physicochemical properties of DNA molecules in aqueous solutions in complexes with methylresorcinol , hexylresorcinol , and tyrosol , the chemical analogs of microbial autoregulators ( d1 factors ) from the group of alkylhydroxybenzenes ( AOB ) , was established .
	manualset3
154039	1	410002	7	NULL	NULL	0	NULL	Izh2p	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that Izh2p can regulate gene expression through this widely dispersed element presents a reasonable explanation of its pleiotropy .
	manualset3
154040	2	410002	7	NULL	NULL	0	NULL	 gene expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that Izh2p can regulate gene expression through this widely dispersed element presents a reasonable explanation of its pleiotropy .
	manualset3
154041	3	410002	7	NULL	NULL	0	NULL	element	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that Izh2p can regulate gene expression through this widely dispersed element presents a reasonable explanation of its pleiotropy .
	manualset3
154042	4	410002	7	NULL	NULL	0	NULL	pleiotropy	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that Izh2p can regulate gene expression through this widely dispersed element presents a reasonable explanation of its pleiotropy .
	manualset3
154074	1	410003	7	NULL	NULL	0	NULL	TRESK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that TRESK is sensitive to volatile anesthetics and localization in central nerve system implies that TRESK may play a very important role in the mechanism mediating general anesthesia .
	manualset3
154075	2	410003	7	NULL	NULL	0	NULL	volatile anesthetics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that TRESK is sensitive to volatile anesthetics and localization in central nerve system implies that TRESK may play a very important role in the mechanism mediating general anesthesia .
	manualset3
154076	4	410003	7	NULL	NULL	NULL	NULL	central nerve system	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fact that TRESK is sensitive to volatile anesthetics and localization in central nerve system implies that TRESK may play a very important role in the mechanism mediating general anesthesia .
	manualset3
154077	5	410003	7	NULL	NULL	NULL	NULL	TRESK	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fact that TRESK is sensitive to volatile anesthetics and localization in central nerve system implies that TRESK may play a very important role in the mechanism mediating general anesthesia .
	manualset3
154078	6	410003	7	NULL	NULL	NULL	NULL	general anesthesia	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fact that TRESK is sensitive to volatile anesthetics and localization in central nerve system implies that TRESK may play a very important role in the mechanism mediating general anesthesia .
	manualset3
154798	3	410003	7	NULL	NULL	0	NULL	localization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that TRESK is sensitive to volatile anesthetics and localization in central nerve system implies that TRESK may play a very important role in the mechanism mediating general anesthesia .
	manualset3
156534	7	410003	7	NULL	NULL	0	NULL	mechanism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that TRESK is sensitive to volatile anesthetics and localization in central nerve system implies that TRESK may play a very important role in the mechanism mediating general anesthesia .
	manualset3
157166	8	410003	7	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that TRESK is sensitive to volatile anesthetics and localization in central nerve system implies that TRESK may play a very important role in the mechanism mediating general anesthesia .
	manualset3
154079	1	410004	7	NULL	NULL	NULL	NULL	quarter of HCV-positive patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fact that a quarter of HCV-positive patients evaluated for a renal transplant have bridging fibrosis or cirrhosis in the liver biopsy may renew renal pre-transplant treatment planning .
	manualset3
154080	2	410004	7	NULL	NULL	0	NULL	 renal transplant	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that a quarter of HCV-positive patients evaluated for a renal transplant have bridging fibrosis or cirrhosis in the liver biopsy may renew renal pre-transplant treatment planning .
	manualset3
154081	3	410004	7	NULL	NULL	0	NULL	fibrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that a quarter of HCV-positive patients evaluated for a renal transplant have bridging fibrosis or cirrhosis in the liver biopsy may renew renal pre-transplant treatment planning .
	manualset3
154082	4	410004	7	NULL	NULL	0	NULL	cirrhosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that a quarter of HCV-positive patients evaluated for a renal transplant have bridging fibrosis or cirrhosis in the liver biopsy may renew renal pre-transplant treatment planning .
	manualset3
154083	5	410004	7	NULL	NULL	0	NULL	 liver biopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that a quarter of HCV-positive patients evaluated for a renal transplant have bridging fibrosis or cirrhosis in the liver biopsy may renew renal pre-transplant treatment planning .
	manualset3
154084	6	410004	7	NULL	NULL	0	NULL	renal pre-transplant treatment planning	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that a quarter of HCV-positive patients evaluated for a renal transplant have bridging fibrosis or cirrhosis in the liver biopsy may renew renal pre-transplant treatment planning .
	manualset3
154094	1	410005	7	NULL	NULL	0	NULL	cytoarchitectonic abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that cytoarchitectonic abnormalities of several types were found in the dreher neocortex may be useful in analyzing the relationship between radial glial fibers and migrating young neurons , the synaptic connections which are formed by ectopically situated neurons , and the mechanism of formation of sporadically distributed neocortical abnormalities .
	manualset3
154095	2	410005	7	NULL	NULL	0	NULL	dreher neocortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that cytoarchitectonic abnormalities of several types were found in the dreher neocortex may be useful in analyzing the relationship between radial glial fibers and migrating young neurons , the synaptic connections which are formed by ectopically situated neurons , and the mechanism of formation of sporadically distributed neocortical abnormalities .
	manualset3
154097	3	410005	7	NULL	NULL	0	NULL	radial glial fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that cytoarchitectonic abnormalities of several types were found in the dreher neocortex may be useful in analyzing the relationship between radial glial fibers and migrating young neurons , the synaptic connections which are formed by ectopically situated neurons , and the mechanism of formation of sporadically distributed neocortical abnormalities .
	manualset3
154098	4	410005	7	NULL	NULL	NULL	NULL	migrating young neurons	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fact that cytoarchitectonic abnormalities of several types were found in the dreher neocortex may be useful in analyzing the relationship between radial glial fibers and migrating young neurons , the synaptic connections which are formed by ectopically situated neurons , and the mechanism of formation of sporadically distributed neocortical abnormalities .
	manualset3
154099	5	410005	7	NULL	NULL	0	NULL	synaptic connections	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that cytoarchitectonic abnormalities of several types were found in the dreher neocortex may be useful in analyzing the relationship between radial glial fibers and migrating young neurons , the synaptic connections which are formed by ectopically situated neurons , and the mechanism of formation of sporadically distributed neocortical abnormalities .
	manualset3
154100	6	410005	7	NULL	NULL	NULL	NULL	ectopically situated neurons	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fact that cytoarchitectonic abnormalities of several types were found in the dreher neocortex may be useful in analyzing the relationship between radial glial fibers and migrating young neurons , the synaptic connections which are formed by ectopically situated neurons , and the mechanism of formation of sporadically distributed neocortical abnormalities .
	manualset3
154101	7	410005	7	NULL	NULL	0	NULL	neocortical abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that cytoarchitectonic abnormalities of several types were found in the dreher neocortex may be useful in analyzing the relationship between radial glial fibers and migrating young neurons , the synaptic connections which are formed by ectopically situated neurons , and the mechanism of formation of sporadically distributed neocortical abnormalities .
	manualset3
154799	8	410005	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that cytoarchitectonic abnormalities of several types were found in the dreher neocortex may be useful in analyzing the relationship between radial glial fibers and migrating young neurons , the synaptic connections which are formed by ectopically situated neurons , and the mechanism of formation of sporadically distributed neocortical abnormalities .
	manualset3
154800	9	410005	7	NULL	NULL	0	NULL	mechanism of formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that cytoarchitectonic abnormalities of several types were found in the dreher neocortex may be useful in analyzing the relationship between radial glial fibers and migrating young neurons , the synaptic connections which are formed by ectopically situated neurons , and the mechanism of formation of sporadically distributed neocortical abnormalities .
	manualset3
157167	10	410005	7	NULL	NULL	0	NULL	 several types	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that cytoarchitectonic abnormalities of several types were found in the dreher neocortex may be useful in analyzing the relationship between radial glial fibers and migrating young neurons , the synaptic connections which are formed by ectopically situated neurons , and the mechanism of formation of sporadically distributed neocortical abnormalities .
	manualset3
154131	1	410006	7	NULL	NULL	0	NULL	insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that insulin improved glucose homeostasis when administrated over a short time period implies that endogenous insulin secretion is inadequate in trout to deal with this amount of dietary carbohydrates .
	manualset3
154132	2	410006	7	NULL	NULL	0	NULL	glucose homeostasis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that insulin improved glucose homeostasis when administrated over a short time period implies that endogenous insulin secretion is inadequate in trout to deal with this amount of dietary carbohydrates .
	manualset3
154133	3	410006	7	NULL	NULL	0	NULL	short time period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that insulin improved glucose homeostasis when administrated over a short time period implies that endogenous insulin secretion is inadequate in trout to deal with this amount of dietary carbohydrates .
	manualset3
154134	4	410006	7	NULL	NULL	NULL	NULL	endogenous insulin secretion	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fact that insulin improved glucose homeostasis when administrated over a short time period implies that endogenous insulin secretion is inadequate in trout to deal with this amount of dietary carbohydrates .
	manualset3
154136	5	410006	7	NULL	NULL	NULL	NULL	trout	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fact that insulin improved glucose homeostasis when administrated over a short time period implies that endogenous insulin secretion is inadequate in trout to deal with this amount of dietary carbohydrates .
	manualset3
154137	6	410006	7	NULL	NULL	NULL	NULL	amount	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fact that insulin improved glucose homeostasis when administrated over a short time period implies that endogenous insulin secretion is inadequate in trout to deal with this amount of dietary carbohydrates .
	manualset3
154138	7	410006	7	NULL	NULL	NULL	NULL	dietary carbohydrates	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fact that insulin improved glucose homeostasis when administrated over a short time period implies that endogenous insulin secretion is inadequate in trout to deal with this amount of dietary carbohydrates .
	manualset3
154139	1	410007	7	NULL	NULL	0	NULL	subgroup	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A subgroup of patients at increased risk of cardiac arrhythmias is defined .
	manualset3
154140	2	410007	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A subgroup of patients at increased risk of cardiac arrhythmias is defined .
	manualset3
154141	3	410007	7	NULL	NULL	NULL	NULL	risk	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A subgroup of patients at increased risk of cardiac arrhythmias is defined .
	manualset3
154142	4	410007	7	NULL	NULL	0	NULL	cardiac arrhythmias	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A subgroup of patients at increased risk of cardiac arrhythmias is defined .
	manualset3
154143	1	410008	7	NULL	NULL	0	NULL	 20 ( S ) - Rg3 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that only 20 ( S ) - Rg3 is active indicates that its hydroxyl group may be geometrically better aligned with the hydroxyl acceptor group in the ion channels than that of 20 ( R ) - Rg3 .
	manualset3
154144	2	410008	7	NULL	NULL	0	NULL	active	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that only 20 ( S ) - Rg3 is active indicates that its hydroxyl group may be geometrically better aligned with the hydroxyl acceptor group in the ion channels than that of 20 ( R ) - Rg3 .
	manualset3
154145	3	410008	7	NULL	NULL	NULL	NULL	hydroxyl group	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fact that only 20 ( S ) - Rg3 is active indicates that its hydroxyl group may be geometrically better aligned with the hydroxyl acceptor group in the ion channels than that of 20 ( R ) - Rg3 .
	manualset3
154146	4	410008	7	NULL	NULL	0	NULL	hydroxyl acceptor group	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that only 20 ( S ) - Rg3 is active indicates that its hydroxyl group may be geometrically better aligned with the hydroxyl acceptor group in the ion channels than that of 20 ( R ) - Rg3 .
	manualset3
154147	5	410008	7	NULL	NULL	0	NULL	ion channels	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that only 20 ( S ) - Rg3 is active indicates that its hydroxyl group may be geometrically better aligned with the hydroxyl acceptor group in the ion channels than that of 20 ( R ) - Rg3 .
	manualset3
154148	6	410008	7	NULL	NULL	0	NULL	20 ( R ) - Rg3	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that only 20 ( S ) - Rg3 is active indicates that its hydroxyl group may be geometrically better aligned with the hydroxyl acceptor group in the ion channels than that of 20 ( R ) - Rg3 .
	manualset3
154149	1	410009	7	NULL	NULL	0	NULL	small children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that some small children understand long and short passives in Portuguese could be seen as evidence that the concept of universal delay for passives is too stringent .
	manualset3
154150	2	410009	7	NULL	NULL	0	NULL	long passives	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that some small children understand long and short passives in Portuguese could be seen as evidence that the concept of universal delay for passives is too stringent .
	manualset3
154151	3	410009	7	NULL	NULL	0	NULL	short passives	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that some small children understand long and short passives in Portuguese could be seen as evidence that the concept of universal delay for passives is too stringent .
	manualset3
154152	4	410009	7	NULL	NULL	0	NULL	Portuguese	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that some small children understand long and short passives in Portuguese could be seen as evidence that the concept of universal delay for passives is too stringent .
	manualset3
154153	5	410009	7	NULL	NULL	0	NULL	concept of universal delay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that some small children understand long and short passives in Portuguese could be seen as evidence that the concept of universal delay for passives is too stringent .
	manualset3
154154	6	410009	7	NULL	NULL	0	NULL	passives	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The fact that some small children understand long and short passives in Portuguese could be seen as evidence that the concept of universal delay for passives is too stringent .
	manualset3
154156	1	410010	7	NULL	NULL	0	NULL	 factor XI inhibitor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The factor XI inhibitor disappeared on day 103 and cardiac catheterization was performed without complications after giving fresh frozen plasma .
	manualset3
154157	2	410010	7	NULL	NULL	0	NULL	day 103	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The factor XI inhibitor disappeared on day 103 and cardiac catheterization was performed without complications after giving fresh frozen plasma .
	manualset3
154158	3	410010	7	NULL	NULL	0	NULL	cardiac catheterization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The factor XI inhibitor disappeared on day 103 and cardiac catheterization was performed without complications after giving fresh frozen plasma .
	manualset3
154159	4	410010	7	NULL	NULL	0	NULL	complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The factor XI inhibitor disappeared on day 103 and cardiac catheterization was performed without complications after giving fresh frozen plasma .
	manualset3
154160	5	410010	7	NULL	NULL	0	NULL	fresh frozen plasma	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The factor XI inhibitor disappeared on day 103 and cardiac catheterization was performed without complications after giving fresh frozen plasma .
	manualset3
154161	1	410011	7	NULL	NULL	NULL	NULL	factors	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The factors required for the generation of memory CD4 T cells remain unclear , and whether there is a continuing requirement for antigen stimulation is critical to design of vaccine strategies .
	manualset3
154162	2	410011	7	NULL	NULL	0	NULL	generation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The factors required for the generation of memory CD4 T cells remain unclear , and whether there is a continuing requirement for antigen stimulation is critical to design of vaccine strategies .
	manualset3
154163	3	410011	7	NULL	NULL	0	NULL	memory CD4 T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The factors required for the generation of memory CD4 T cells remain unclear , and whether there is a continuing requirement for antigen stimulation is critical to design of vaccine strategies .
	manualset3
154164	4	410011	7	NULL	NULL	0	NULL	antigen stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The factors required for the generation of memory CD4 T cells remain unclear , and whether there is a continuing requirement for antigen stimulation is critical to design of vaccine strategies .
	manualset3
154165	5	410011	7	NULL	NULL	0	NULL	vaccine strategies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The factors required for the generation of memory CD4 T cells remain unclear , and whether there is a continuing requirement for antigen stimulation is critical to design of vaccine strategies .
	manualset3
157168	6	410011	7	NULL	NULL	0	NULL	requirement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The factors required for the generation of memory CD4 T cells remain unclear , and whether there is a continuing requirement for antigen stimulation is critical to design of vaccine strategies .
	manualset3
154166	1	410012	7	NULL	NULL	0	NULL	factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The factors that led to a greater rate of complications were the severity of neurologic involvement , severity of recent history of significant medical problems , and severity of scoliosis .
	manualset3
154167	2	410012	7	NULL	NULL	NULL	NULL	greater rate of complications	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The factors that led to a greater rate of complications were the severity of neurologic involvement , severity of recent history of significant medical problems , and severity of scoliosis .
	manualset3
154168	3	410012	7	NULL	NULL	NULL	NULL	severity of neurologic involvement	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The factors that led to a greater rate of complications were the severity of neurologic involvement , severity of recent history of significant medical problems , and severity of scoliosis .
	manualset3
154170	4	410012	7	NULL	NULL	NULL	NULL	severity of recent history of significant medical problems	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The factors that led to a greater rate of complications were the severity of neurologic involvement , severity of recent history of significant medical problems , and severity of scoliosis .
	manualset3
154171	5	410012	7	NULL	NULL	NULL	NULL	severity of scoliosis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The factors that led to a greater rate of complications were the severity of neurologic involvement , severity of recent history of significant medical problems , and severity of scoliosis .
	manualset3
154172	1	410013	7	NULL	NULL	0	NULL	 factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The factors under investigation were : binder grade , mixer load , presence of the deflector ( all of analyzed at two levels ) , binder concentration , impeller speed , massing time , type of impeller blades ( these four at three levels ) and jacket temperature ( considered at four levels ) .
	manualset3
154173	2	410013	7	NULL	NULL	0	NULL	investigation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The factors under investigation were : binder grade , mixer load , presence of the deflector ( all of analyzed at two levels ) , binder concentration , impeller speed , massing time , type of impeller blades ( these four at three levels ) and jacket temperature ( considered at four levels ) .
	manualset3
154174	3	410013	7	NULL	NULL	0	NULL	binder grade	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The factors under investigation were : binder grade , mixer load , presence of the deflector ( all of analyzed at two levels ) , binder concentration , impeller speed , massing time , type of impeller blades ( these four at three levels ) and jacket temperature ( considered at four levels ) .
	manualset3
154175	4	410013	7	NULL	NULL	0	NULL	mixer load	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The factors under investigation were : binder grade , mixer load , presence of the deflector ( all of analyzed at two levels ) , binder concentration , impeller speed , massing time , type of impeller blades ( these four at three levels ) and jacket temperature ( considered at four levels ) .
	manualset3
154176	5	410013	7	NULL	NULL	0	NULL	deflector ( all of analyzed at two levels )	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The factors under investigation were : binder grade , mixer load , presence of the deflector ( all of analyzed at two levels ) , binder concentration , impeller speed , massing time , type of impeller blades ( these four at three levels ) and jacket temperature ( considered at four levels ) .
	manualset3
154177	6	410013	7	NULL	NULL	0	NULL	binder concentration	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The factors under investigation were : binder grade , mixer load , presence of the deflector ( all of analyzed at two levels ) , binder concentration , impeller speed , massing time , type of impeller blades ( these four at three levels ) and jacket temperature ( considered at four levels ) .
	manualset3
154178	7	410013	7	NULL	NULL	0	NULL	impeller speed	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The factors under investigation were : binder grade , mixer load , presence of the deflector ( all of analyzed at two levels ) , binder concentration , impeller speed , massing time , type of impeller blades ( these four at three levels ) and jacket temperature ( considered at four levels ) .
	manualset3
154179	8	410013	7	NULL	NULL	0	NULL	massing time	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The factors under investigation were : binder grade , mixer load , presence of the deflector ( all of analyzed at two levels ) , binder concentration , impeller speed , massing time , type of impeller blades ( these four at three levels ) and jacket temperature ( considered at four levels ) .
	manualset3
154180	9	410013	7	NULL	NULL	0	NULL	impeller blades	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The factors under investigation were : binder grade , mixer load , presence of the deflector ( all of analyzed at two levels ) , binder concentration , impeller speed , massing time , type of impeller blades ( these four at three levels ) and jacket temperature ( considered at four levels ) .
	manualset3
154181	10	410013	7	NULL	NULL	NULL	NULL	 four at three levels 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The factors under investigation were : binder grade , mixer load , presence of the deflector ( all of analyzed at two levels ) , binder concentration , impeller speed , massing time , type of impeller blades ( these four at three levels ) and jacket temperature ( considered at four levels ) .
	manualset3
154182	11	410013	7	NULL	NULL	0	NULL	jacket temperature	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The factors under investigation were : binder grade , mixer load , presence of the deflector ( all of analyzed at two levels ) , binder concentration , impeller speed , massing time , type of impeller blades ( these four at three levels ) and jacket temperature ( considered at four levels ) .
	manualset3
154183	12	410013	7	NULL	NULL	NULL	NULL	four levels	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The factors under investigation were : binder grade , mixer load , presence of the deflector ( all of analyzed at two levels ) , binder concentration , impeller speed , massing time , type of impeller blades ( these four at three levels ) and jacket temperature ( considered at four levels ) .
	manualset3
154261	1	410014	7	NULL	NULL	0	NULL	 factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The factors with the greatest influence on the use of rescue medication were the analgesic taken by the patient and the presence or not of postoperative inflammation .
	manualset3
154263	2	410014	7	NULL	NULL	0	NULL	rescue medication	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The factors with the greatest influence on the use of rescue medication were the analgesic taken by the patient and the presence or not of postoperative inflammation .
	manualset3
154264	3	410014	7	NULL	NULL	0	NULL	analgesic	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The factors with the greatest influence on the use of rescue medication were the analgesic taken by the patient and the presence or not of postoperative inflammation .
	manualset3
154266	4	410014	7	NULL	NULL	0	NULL	patient	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The factors with the greatest influence on the use of rescue medication were the analgesic taken by the patient and the presence or not of postoperative inflammation .
	manualset3
154274	5	410014	7	NULL	NULL	0	NULL	postoperative inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The factors with the greatest influence on the use of rescue medication were the analgesic taken by the patient and the presence or not of postoperative inflammation .
	manualset3
157169	6	410014	7	NULL	NULL	0	NULL	influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The factors with the greatest influence on the use of rescue medication were the analgesic taken by the patient and the presence or not of postoperative inflammation .
	manualset3
157170	7	410014	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The factors with the greatest influence on the use of rescue medication were the analgesic taken by the patient and the presence or not of postoperative inflammation .
	manualset3
154278	1	410015	7	NULL	NULL	NULL	NULL	failure of STZ 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The failure of STZ to cure tumor-bearing mice was next addressed considering three possible mechanisms : ( a ) STZ was less tumoricidal ; ( b ) STZ suppressed the immunity of the host ; and ( c ) STZ failed to eliminate tumor-specific suppressor T-cells .
	manualset3
154283	2	410015	7	NULL	NULL	NULL	NULL	 tumor-bearing mice	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The failure of STZ to cure tumor-bearing mice was next addressed considering three possible mechanisms : ( a ) STZ was less tumoricidal ; ( b ) STZ suppressed the immunity of the host ; and ( c ) STZ failed to eliminate tumor-specific suppressor T-cells .
	manualset3
154287	3	410015	7	NULL	NULL	NULL	NULL	immunity of the host	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The failure of STZ to cure tumor-bearing mice was next addressed considering three possible mechanisms : ( a ) STZ was less tumoricidal ; ( b ) STZ suppressed the immunity of the host ; and ( c ) STZ failed to eliminate tumor-specific suppressor T-cells .
	manualset3
154289	4	410015	7	NULL	NULL	NULL	NULL	tumor-specific suppressor T-cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The failure of STZ to cure tumor-bearing mice was next addressed considering three possible mechanisms : ( a ) STZ was less tumoricidal ; ( b ) STZ suppressed the immunity of the host ; and ( c ) STZ failed to eliminate tumor-specific suppressor T-cells .
	manualset3
154291	5	410015	7	NULL	NULL	NULL	NULL	three possible mechanisms	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The failure of STZ to cure tumor-bearing mice was next addressed considering three possible mechanisms : ( a ) STZ was less tumoricidal ; ( b ) STZ suppressed the immunity of the host ; and ( c ) STZ failed to eliminate tumor-specific suppressor T-cells .
	manualset3
154866	6	410015	7	NULL	NULL	0	NULL	STZ 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The failure of STZ to cure tumor-bearing mice was next addressed considering three possible mechanisms : ( a ) STZ was less tumoricidal ; ( b ) STZ suppressed the immunity of the host ; and ( c ) STZ failed to eliminate tumor-specific suppressor T-cells .
	manualset3
157171	7	410015	7	NULL	NULL	NULL	NULL	STZ	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The failure of STZ to cure tumor-bearing mice was next addressed considering three possible mechanisms : ( a ) STZ was less tumoricidal ; ( b ) STZ suppressed the immunity of the host ; and ( c ) STZ failed to eliminate tumor-specific suppressor T-cells .
	manualset3
157172	8	410015	7	NULL	NULL	0	NULL	STZ	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The failure of STZ to cure tumor-bearing mice was next addressed considering three possible mechanisms : ( a ) STZ was less tumoricidal ; ( b ) STZ suppressed the immunity of the host ; and ( c ) STZ failed to eliminate tumor-specific suppressor T-cells .
	manualset3
154302	1	410016	7	NULL	NULL	0	NULL	 failure of the Guggenheim model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The failure of the Guggenheim model is also evident in our calculations for water-methanol , water-ethanol , and water-n-propanol mixtures .
	manualset3
154303	2	410016	7	NULL	NULL	0	NULL	calculations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The failure of the Guggenheim model is also evident in our calculations for water-methanol , water-ethanol , and water-n-propanol mixtures .
	manualset3
154304	3	410016	7	NULL	NULL	0	NULL	 water-methanol mixture	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The failure of the Guggenheim model is also evident in our calculations for water-methanol , water-ethanol , and water-n-propanol mixtures .
	manualset3
154305	4	410016	7	NULL	NULL	0	NULL	water-ethanol mixture	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The failure of the Guggenheim model is also evident in our calculations for water-methanol , water-ethanol , and water-n-propanol mixtures .
	manualset3
154306	5	410016	7	NULL	NULL	0	NULL	water-n-propanol mixture	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The failure of the Guggenheim model is also evident in our calculations for water-methanol , water-ethanol , and water-n-propanol mixtures .
	manualset3
154307	1	410017	7	NULL	NULL	0	NULL	failure 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The failure to detect formation of radioactive 1 , 25 - ( OH ) 2D3 in vitamin D-replete subjects suggests that current estimates of the daily turnover of the hormone in the normal individual may be severalfold too high .
	manualset3
154308	2	410017	7	NULL	NULL	0	NULL	formation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The failure to detect formation of radioactive 1 , 25 - ( OH ) 2D3 in vitamin D-replete subjects suggests that current estimates of the daily turnover of the hormone in the normal individual may be severalfold too high .
	manualset3
154309	3	410017	7	NULL	NULL	0	NULL	radioactive 1 , 25 - ( OH ) 2D3	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The failure to detect formation of radioactive 1 , 25 - ( OH ) 2D3 in vitamin D-replete subjects suggests that current estimates of the daily turnover of the hormone in the normal individual may be severalfold too high .
	manualset3
154310	4	410017	7	NULL	NULL	0	NULL	 vitamin D-replete subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The failure to detect formation of radioactive 1 , 25 - ( OH ) 2D3 in vitamin D-replete subjects suggests that current estimates of the daily turnover of the hormone in the normal individual may be severalfold too high .
	manualset3
154311	5	410017	7	NULL	NULL	0	NULL	current estimates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The failure to detect formation of radioactive 1 , 25 - ( OH ) 2D3 in vitamin D-replete subjects suggests that current estimates of the daily turnover of the hormone in the normal individual may be severalfold too high .
	manualset3
154312	6	410017	7	NULL	NULL	0	NULL	daily turnover 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The failure to detect formation of radioactive 1 , 25 - ( OH ) 2D3 in vitamin D-replete subjects suggests that current estimates of the daily turnover of the hormone in the normal individual may be severalfold too high .
	manualset3
154313	7	410017	7	NULL	NULL	0	NULL	hormone	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The failure to detect formation of radioactive 1 , 25 - ( OH ) 2D3 in vitamin D-replete subjects suggests that current estimates of the daily turnover of the hormone in the normal individual may be severalfold too high .
	manualset3
154314	8	410017	7	NULL	NULL	0	NULL	normal individual 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The failure to detect formation of radioactive 1 , 25 - ( OH ) 2D3 in vitamin D-replete subjects suggests that current estimates of the daily turnover of the hormone in the normal individual may be severalfold too high .
	manualset3
154344	1	410018	7	NULL	NULL	0	NULL	subgroup of patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A subgroup of patients in each group were tested for gustatory sweating ( iodine starch test ) and parotid function ( quantitative scintigraphy ) .
	manualset3
154345	2	410018	7	NULL	NULL	0	NULL	group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A subgroup of patients in each group were tested for gustatory sweating ( iodine starch test ) and parotid function ( quantitative scintigraphy ) .
	manualset3
154346	3	410018	7	NULL	NULL	0	NULL	gustatory sweating 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A subgroup of patients in each group were tested for gustatory sweating ( iodine starch test ) and parotid function ( quantitative scintigraphy ) .
	manualset3
154347	4	410018	7	NULL	NULL	0	NULL	 iodine starch test	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A subgroup of patients in each group were tested for gustatory sweating ( iodine starch test ) and parotid function ( quantitative scintigraphy ) .
	manualset3
154348	5	410018	7	NULL	NULL	0	NULL	parotid function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A subgroup of patients in each group were tested for gustatory sweating ( iodine starch test ) and parotid function ( quantitative scintigraphy ) .
	manualset3
154349	6	410018	7	NULL	NULL	0	NULL	quantitative scintigraphy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A subgroup of patients in each group were tested for gustatory sweating ( iodine starch test ) and parotid function ( quantitative scintigraphy ) .
	manualset3
154350	1	410019	7	NULL	NULL	0	NULL	 failure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The failure to improve the five-year survival rate of cancer patients , from one in three in the 1960s to one in two in the 1970s , stimulated awareness of the importance of primary prevention of cancer .
	manualset3
154351	2	410019	7	NULL	NULL	NULL	NULL	five-year survival rate 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The failure to improve the five-year survival rate of cancer patients , from one in three in the 1960s to one in two in the 1970s , stimulated awareness of the importance of primary prevention of cancer .
	manualset3
154352	3	410019	7	NULL	NULL	NULL	NULL	cancer patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The failure to improve the five-year survival rate of cancer patients , from one in three in the 1960s to one in two in the 1970s , stimulated awareness of the importance of primary prevention of cancer .
	manualset3
154353	4	410019	7	NULL	NULL	0	NULL	1960s	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The failure to improve the five-year survival rate of cancer patients , from one in three in the 1960s to one in two in the 1970s , stimulated awareness of the importance of primary prevention of cancer .
	manualset3
154354	5	410019	7	NULL	NULL	0	NULL	1970s	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The failure to improve the five-year survival rate of cancer patients , from one in three in the 1960s to one in two in the 1970s , stimulated awareness of the importance of primary prevention of cancer .
	manualset3
154355	6	410019	7	NULL	NULL	0	NULL	primary prevention 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The failure to improve the five-year survival rate of cancer patients , from one in three in the 1960s to one in two in the 1970s , stimulated awareness of the importance of primary prevention of cancer .
	manualset3
154356	7	410019	7	NULL	NULL	0	NULL	cancer	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The failure to improve the five-year survival rate of cancer patients , from one in three in the 1960s to one in two in the 1970s , stimulated awareness of the importance of primary prevention of cancer .
	manualset3
157173	8	410019	7	NULL	NULL	0	NULL	one in three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The failure to improve the five-year survival rate of cancer patients , from one in three in the 1960s to one in two in the 1970s , stimulated awareness of the importance of primary prevention of cancer .
	manualset3
157174	9	410019	7	NULL	NULL	0	NULL	one in two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The failure to improve the five-year survival rate of cancer patients , from one in three in the 1960s to one in two in the 1970s , stimulated awareness of the importance of primary prevention of cancer .
	manualset3
157175	10	410019	7	NULL	NULL	0	NULL	awareness	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The failure to improve the five-year survival rate of cancer patients , from one in three in the 1960s to one in two in the 1970s , stimulated awareness of the importance of primary prevention of cancer .
	manualset3
157176	11	410019	7	NULL	NULL	0	NULL	importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The failure to improve the five-year survival rate of cancer patients , from one in three in the 1960s to one in two in the 1970s , stimulated awareness of the importance of primary prevention of cancer .
	manualset3
154357	1	410020	7	NULL	NULL	NULL	NULL	fair use	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fair use of lower-limb running prostheses : A Delphi study .
	manualset3
154358	2	410020	7	NULL	NULL	NULL	NULL	lower-limb  running prostheses	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fair use of lower-limb running prostheses : A Delphi study .
	manualset3
154360	3	410020	7	NULL	NULL	NULL	NULL	A Delphi study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fair use of lower-limb running prostheses : A Delphi study .
	manualset3
154362	1	410021	7	NULL	NULL	NULL	NULL	fall of blood pressure	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fall of blood pressure is accompanied by an increase in heart rate and cardiac output and a decrease in total peripheral resistance .
	manualset3
154363	2	410021	7	NULL	NULL	NULL	NULL	increase in heart rate	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fall of blood pressure is accompanied by an increase in heart rate and cardiac output and a decrease in total peripheral resistance .
	manualset3
154364	3	410021	7	NULL	NULL	NULL	NULL	increase in cardiac output 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fall of blood pressure is accompanied by an increase in heart rate and cardiac output and a decrease in total peripheral resistance .
	manualset3
154365	4	410021	7	NULL	NULL	NULL	NULL	decrease in total peripheral resistance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fall of blood pressure is accompanied by an increase in heart rate and cardiac output and a decrease in total peripheral resistance .
	manualset3
154366	1	410022	7	NULL	NULL	0	NULL	family Hyphomonadaceae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The family Hyphomonadaceae within the Alphaproteobacteria is largely comprised of bacteria isolated from marine environments with striking morphologies and an unusual mode of cell growth .
	manualset3
154367	2	410022	7	NULL	NULL	0	NULL	Alphaproteobacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The family Hyphomonadaceae within the Alphaproteobacteria is largely comprised of bacteria isolated from marine environments with striking morphologies and an unusual mode of cell growth .
	manualset3
154368	3	410022	7	NULL	NULL	0	NULL	bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The family Hyphomonadaceae within the Alphaproteobacteria is largely comprised of bacteria isolated from marine environments with striking morphologies and an unusual mode of cell growth .
	manualset3
154369	4	410022	7	NULL	NULL	0	NULL	marine environments 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The family Hyphomonadaceae within the Alphaproteobacteria is largely comprised of bacteria isolated from marine environments with striking morphologies and an unusual mode of cell growth .
	manualset3
154370	5	410022	7	NULL	NULL	0	NULL	morphologies	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The family Hyphomonadaceae within the Alphaproteobacteria is largely comprised of bacteria isolated from marine environments with striking morphologies and an unusual mode of cell growth .
	manualset3
154371	6	410022	7	NULL	NULL	0	NULL	cell growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The family Hyphomonadaceae within the Alphaproteobacteria is largely comprised of bacteria isolated from marine environments with striking morphologies and an unusual mode of cell growth .
	manualset3
157177	7	410022	7	NULL	NULL	0	NULL	unusual mode	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The family Hyphomonadaceae within the Alphaproteobacteria is largely comprised of bacteria isolated from marine environments with striking morphologies and an unusual mode of cell growth .
	manualset3
154372	1	410023	7	NULL	NULL	0	NULL	family	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The family was identified through the analysis of M81 , a mating-induced gene .
	manualset3
154373	2	410023	7	NULL	NULL	0	NULL	M81	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The family was identified through the analysis of M81 , a mating-induced gene .
	manualset3
154374	3	410023	7	NULL	NULL	0	NULL	mating-induced gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The family was identified through the analysis of M81 , a mating-induced gene .
	manualset3
157178	4	410023	7	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The family was identified through the analysis of M81 , a mating-induced gene .
	manualset3
154375	1	410024	7	NULL	NULL	0	NULL	farmers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The farmers recorded the favored resting location of the individual cows and heifers throughout the final week of pregnancy as well as during calving .
	manualset3
154376	2	410024	7	NULL	NULL	NULL	NULL	favored resting location	GeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The farmers recorded the favored resting location of the individual cows and heifers throughout the final week of pregnancy as well as during calving .
	manualset3
154377	3	410024	7	NULL	NULL	0	NULL	 individual cows	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The farmers recorded the favored resting location of the individual cows and heifers throughout the final week of pregnancy as well as during calving .
	manualset3
154378	4	410024	7	NULL	NULL	0	NULL	heifers	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The farmers recorded the favored resting location of the individual cows and heifers throughout the final week of pregnancy as well as during calving .
	manualset3
154379	5	410024	7	NULL	NULL	NULL	NULL	final week of pregnancy	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The farmers recorded the favored resting location of the individual cows and heifers throughout the final week of pregnancy as well as during calving .
	manualset3
154380	1	410025	7	NULL	NULL	0	NULL	fasting	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The fasting had little effect on the lipid patterns of the various types of muscles except for those of phospholipids in heart muscle .
	manualset3
154381	2	410025	7	NULL	NULL	0	NULL	little effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The fasting had little effect on the lipid patterns of the various types of muscles except for those of phospholipids in heart muscle .
	manualset3
154382	3	410025	7	NULL	NULL	0	NULL	lipid patterns	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The fasting had little effect on the lipid patterns of the various types of muscles except for those of phospholipids in heart muscle .
	manualset3
154383	4	410025	7	NULL	NULL	0	NULL	types of muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The fasting had little effect on the lipid patterns of the various types of muscles except for those of phospholipids in heart muscle .
	manualset3
154384	5	410025	7	NULL	NULL	0	NULL	phospholipids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The fasting had little effect on the lipid patterns of the various types of muscles except for those of phospholipids in heart muscle .
	manualset3
154385	6	410025	7	NULL	NULL	0	NULL	heart muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The fasting had little effect on the lipid patterns of the various types of muscles except for those of phospholipids in heart muscle .
	manualset3
154386	1	410026	7	NULL	NULL	0	NULL	fatal potential	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The fatal potential of fistula-in-ano with abscess : analysis of 11 deaths .
	manualset3
154387	2	410026	7	NULL	NULL	0	NULL	fistula-in-ano with abscess	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The fatal potential of fistula-in-ano with abscess : analysis of 11 deaths .
	manualset3
154388	3	410026	7	NULL	NULL	NULL	NULL	analysis of 11 deaths	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fatal potential of fistula-in-ano with abscess : analysis of 11 deaths .
	manualset3
154389	1	410027	7	NULL	NULL	NULL	NULL	subject 's response	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A subject 's response to chromium depends on his or her chromium status , diet consumed , type and amount of supplemental chromium , and study duration .
	manualset3
154390	2	410027	7	NULL	NULL	0	NULL	chromium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A subject 's response to chromium depends on his or her chromium status , diet consumed , type and amount of supplemental chromium , and study duration .
	manualset3
154391	3	410027	7	NULL	NULL	0	NULL	chromium status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A subject 's response to chromium depends on his or her chromium status , diet consumed , type and amount of supplemental chromium , and study duration .
	manualset3
154392	4	410027	7	NULL	NULL	0	NULL	 diet consumed 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A subject 's response to chromium depends on his or her chromium status , diet consumed , type and amount of supplemental chromium , and study duration .
	manualset3
154393	5	410027	7	NULL	NULL	0	NULL	type and amount of supplemental chromium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A subject 's response to chromium depends on his or her chromium status , diet consumed , type and amount of supplemental chromium , and study duration .
	manualset3
154394	6	410027	7	NULL	NULL	NULL	NULL	study duration	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A subject 's response to chromium depends on his or her chromium status , diet consumed , type and amount of supplemental chromium , and study duration .
	manualset3
154396	1	410028	7	NULL	NULL	0	NULL	fate 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The fate of alpha and epsilon lysine amino groups has been explored in rat liver homogenate by means of L-lysine labeled selectively in the two positions .
	manualset3
154398	2	410028	7	NULL	NULL	0	NULL	alpha lysine amino groups	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The fate of alpha and epsilon lysine amino groups has been explored in rat liver homogenate by means of L-lysine labeled selectively in the two positions .
	manualset3
154399	3	410028	7	NULL	NULL	0	NULL	epsilon lysine amino groups	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The fate of alpha and epsilon lysine amino groups has been explored in rat liver homogenate by means of L-lysine labeled selectively in the two positions .
	manualset3
154400	4	410028	7	NULL	NULL	NULL	NULL	rat liver homogenate	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fate of alpha and epsilon lysine amino groups has been explored in rat liver homogenate by means of L-lysine labeled selectively in the two positions .
	manualset3
154401	5	410028	7	NULL	NULL	0	NULL	L-lysine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The fate of alpha and epsilon lysine amino groups has been explored in rat liver homogenate by means of L-lysine labeled selectively in the two positions .
	manualset3
154402	6	410028	7	NULL	NULL	NULL	NULL	two positions	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fate of alpha and epsilon lysine amino groups has been explored in rat liver homogenate by means of L-lysine labeled selectively in the two positions .
	manualset3
154403	1	410029	7	NULL	NULL	NULL	NULL	fate	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fate of endogenous stem cells in the brain was examined by the expression of the stem cell marker nestin , together with Tf , neurofilaments and glial fibrillary acidic protein from 2 to 14 days after injection .
	manualset3
154404	2	410029	7	NULL	NULL	0	NULL	endogenous stem cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The fate of endogenous stem cells in the brain was examined by the expression of the stem cell marker nestin , together with Tf , neurofilaments and glial fibrillary acidic protein from 2 to 14 days after injection .
	manualset3
154405	3	410029	7	NULL	NULL	0	NULL	 brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The fate of endogenous stem cells in the brain was examined by the expression of the stem cell marker nestin , together with Tf , neurofilaments and glial fibrillary acidic protein from 2 to 14 days after injection .
	manualset3
154406	4	410029	7	NULL	NULL	NULL	NULL	expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fate of endogenous stem cells in the brain was examined by the expression of the stem cell marker nestin , together with Tf , neurofilaments and glial fibrillary acidic protein from 2 to 14 days after injection .
	manualset3
154407	5	410029	7	NULL	NULL	0	NULL	stem cell marker nestin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The fate of endogenous stem cells in the brain was examined by the expression of the stem cell marker nestin , together with Tf , neurofilaments and glial fibrillary acidic protein from 2 to 14 days after injection .
	manualset3
154408	6	410029	7	NULL	NULL	0	NULL	Tf	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The fate of endogenous stem cells in the brain was examined by the expression of the stem cell marker nestin , together with Tf , neurofilaments and glial fibrillary acidic protein from 2 to 14 days after injection .
	manualset3
154409	7	410029	7	NULL	NULL	0	NULL	neurofilaments	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The fate of endogenous stem cells in the brain was examined by the expression of the stem cell marker nestin , together with Tf , neurofilaments and glial fibrillary acidic protein from 2 to 14 days after injection .
	manualset3
154410	8	410029	7	NULL	NULL	0	NULL	glial fibrillary acidic protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The fate of endogenous stem cells in the brain was examined by the expression of the stem cell marker nestin , together with Tf , neurofilaments and glial fibrillary acidic protein from 2 to 14 days after injection .
	manualset3
154411	9	410029	7	NULL	NULL	0	NULL	2 to 14 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The fate of endogenous stem cells in the brain was examined by the expression of the stem cell marker nestin , together with Tf , neurofilaments and glial fibrillary acidic protein from 2 to 14 days after injection .
	manualset3
154412	10	410029	7	NULL	NULL	0	NULL	injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The fate of endogenous stem cells in the brain was examined by the expression of the stem cell marker nestin , together with Tf , neurofilaments and glial fibrillary acidic protein from 2 to 14 days after injection .
	manualset3
154413	1	410030	7	NULL	NULL	0	NULL	fate 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The fate of the endothelial cells of the graft as determined by sex chromatin studies .
	manualset3
154414	2	410030	7	NULL	NULL	0	NULL	endothelial cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The fate of the endothelial cells of the graft as determined by sex chromatin studies .
	manualset3
154415	3	410030	7	NULL	NULL	0	NULL	graft 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The fate of the endothelial cells of the graft as determined by sex chromatin studies .
	manualset3
154416	4	410030	7	NULL	NULL	0	NULL	sex chromatin studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The fate of the endothelial cells of the graft as determined by sex chromatin studies .
	manualset3
154962	1	410031	7	NULL	NULL	0	NULL	favorable results	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The favorable results of the research suggested a potential feasibility of MAT-MI in electrical impedance imaging .
	manualset3
154963	2	410031	7	NULL	NULL	0	NULL	 research`	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The favorable results of the research suggested a potential feasibility of MAT-MI in electrical impedance imaging .
	manualset3
154964	3	410031	7	NULL	NULL	0	NULL	potential feasibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The favorable results of the research suggested a potential feasibility of MAT-MI in electrical impedance imaging .
	manualset3
154965	4	410031	7	NULL	NULL	NULL	NULL	MAT-MI	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The favorable results of the research suggested a potential feasibility of MAT-MI in electrical impedance imaging .
	manualset3
154966	5	410031	7	NULL	NULL	0	NULL	electrical impedance imaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The favorable results of the research suggested a potential feasibility of MAT-MI in electrical impedance imaging .
	manualset3
154967	1	410032	7	NULL	NULL	0	NULL	 feature vector 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The feature vector is based on the linear prediction coefficients of the autoregressive method after an adaptive line enhancement method was used as the input pattern to the neural network .
	manualset3
154968	2	410032	7	NULL	NULL	0	NULL	linear prediction coefficients	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The feature vector is based on the linear prediction coefficients of the autoregressive method after an adaptive line enhancement method was used as the input pattern to the neural network .
	manualset3
154969	3	410032	7	NULL	NULL	0	NULL	autoregressive method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The feature vector is based on the linear prediction coefficients of the autoregressive method after an adaptive line enhancement method was used as the input pattern to the neural network .
	manualset3
154970	4	410032	7	NULL	NULL	0	NULL	adaptive line enhancement method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The feature vector is based on the linear prediction coefficients of the autoregressive method after an adaptive line enhancement method was used as the input pattern to the neural network .
	manualset3
154971	5	410032	7	NULL	NULL	0	NULL	 input pattern	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The feature vector is based on the linear prediction coefficients of the autoregressive method after an adaptive line enhancement method was used as the input pattern to the neural network .
	manualset3
154972	6	410032	7	NULL	NULL	0	NULL	neural network	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The feature vector is based on the linear prediction coefficients of the autoregressive method after an adaptive line enhancement method was used as the input pattern to the neural network .
	manualset3
154973	1	410033	7	NULL	NULL	0	NULL	fecal weights of mice	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The fecal weights of mice were increased by the high-fat diet containing EPL compared with the high-fat diet alone .
	manualset3
154974	2	410033	7	NULL	NULL	0	NULL	 high-fat diet 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The fecal weights of mice were increased by the high-fat diet containing EPL compared with the high-fat diet alone .
	manualset3
154975	3	410033	7	NULL	NULL	0	NULL	EPL	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The fecal weights of mice were increased by the high-fat diet containing EPL compared with the high-fat diet alone .
	manualset3
154976	4	410033	7	NULL	NULL	0	NULL	high-fat diet 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The fecal weights of mice were increased by the high-fat diet containing EPL compared with the high-fat diet alone .
	manualset3
154977	1	410034	7	NULL	NULL	0	NULL	female gametophyte	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The female gametophyte exerts control over the male , with specialized cells known as synergids guiding the pollen tubes and controlling their behavior when they enter the female gametophyte so that the sperm cells can be delivered to the egg and central cell .
	manualset3
154978	2	410034	7	NULL	NULL	0	NULL	male	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The female gametophyte exerts control over the male , with specialized cells known as synergids guiding the pollen tubes and controlling their behavior when they enter the female gametophyte so that the sperm cells can be delivered to the egg and central cell .
	manualset3
154979	3	410034	7	NULL	NULL	0	NULL	specialized cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The female gametophyte exerts control over the male , with specialized cells known as synergids guiding the pollen tubes and controlling their behavior when they enter the female gametophyte so that the sperm cells can be delivered to the egg and central cell .
	manualset3
154980	4	410034	7	NULL	NULL	0	NULL	synergids	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The female gametophyte exerts control over the male , with specialized cells known as synergids guiding the pollen tubes and controlling their behavior when they enter the female gametophyte so that the sperm cells can be delivered to the egg and central cell .
	manualset3
154981	5	410034	7	NULL	NULL	0	NULL	pollen tubes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The female gametophyte exerts control over the male , with specialized cells known as synergids guiding the pollen tubes and controlling their behavior when they enter the female gametophyte so that the sperm cells can be delivered to the egg and central cell .
	manualset3
154982	6	410034	7	NULL	NULL	0	NULL	female gametophyte	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The female gametophyte exerts control over the male , with specialized cells known as synergids guiding the pollen tubes and controlling their behavior when they enter the female gametophyte so that the sperm cells can be delivered to the egg and central cell .
	manualset3
154983	7	410034	7	NULL	NULL	0	NULL	sperm cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The female gametophyte exerts control over the male , with specialized cells known as synergids guiding the pollen tubes and controlling their behavior when they enter the female gametophyte so that the sperm cells can be delivered to the egg and central cell .
	manualset3
154984	8	410034	7	NULL	NULL	0	NULL	egg 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The female gametophyte exerts control over the male , with specialized cells known as synergids guiding the pollen tubes and controlling their behavior when they enter the female gametophyte so that the sperm cells can be delivered to the egg and central cell .
	manualset3
154985	9	410034	7	NULL	NULL	0	NULL	central cell 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The female gametophyte exerts control over the male , with specialized cells known as synergids guiding the pollen tubes and controlling their behavior when they enter the female gametophyte so that the sperm cells can be delivered to the egg and central cell .
	manualset3
157273	10	410034	7	NULL	NULL	0	NULL	behavior	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The female gametophyte exerts control over the male , with specialized cells known as synergids guiding the pollen tubes and controlling their behavior when they enter the female gametophyte so that the sperm cells can be delivered to the egg and central cell .
	manualset3
154986	1	410035	7	NULL	NULL	0	NULL	fermentation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The fermentation , isolation , structure elucidation and some properties are described .
	manualset3
154987	2	410035	7	NULL	NULL	NULL	NULL	isolation	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fermentation , isolation , structure elucidation and some properties are described .
	manualset3
154988	3	410035	7	NULL	NULL	0	NULL	structure elucidation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The fermentation , isolation , structure elucidation and some properties are described .
	manualset3
154989	4	410035	7	NULL	NULL	0	NULL	properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The fermentation , isolation , structure elucidation and some properties are described .
	manualset3
154990	1	410036	7	NULL	NULL	0	NULL	fermentation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The fermentation performed by forced pH fluctuations with pH = 1.0 , risen at every 3h was evaluated as the most successful .
	manualset3
154991	2	410036	7	NULL	NULL	0	NULL	forced pH fluctuations	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The fermentation performed by forced pH fluctuations with pH = 1.0 , risen at every 3h was evaluated as the most successful .
	manualset3
154992	3	410036	7	NULL	NULL	0	NULL	pH = 1.0	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The fermentation performed by forced pH fluctuations with pH = 1.0 , risen at every 3h was evaluated as the most successful .
	manualset3
154993	4	410036	7	NULL	NULL	0	NULL	3h	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The fermentation performed by forced pH fluctuations with pH = 1.0 , risen at every 3h was evaluated as the most successful .
	manualset3
154994	1	410037	7	NULL	NULL	0	NULL	ferredoxin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ferredoxin from the thermophilic archaeon Acidianus ambivalens is a small monomeric seven-iron protein with a thermal midpoint ( T ( m ) ) of 122 degrees C ( pH 7 ) .
	manualset3
154995	2	410037	7	NULL	NULL	0	NULL	thermophilic archaeon Acidianus ambivalens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The ferredoxin from the thermophilic archaeon Acidianus ambivalens is a small monomeric seven-iron protein with a thermal midpoint ( T ( m ) ) of 122 degrees C ( pH 7 ) .
	manualset3
154996	3	410037	7	NULL	NULL	0	NULL	small monomeric seven-iron protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The ferredoxin from the thermophilic archaeon Acidianus ambivalens is a small monomeric seven-iron protein with a thermal midpoint ( T ( m ) ) of 122 degrees C ( pH 7 ) .
	manualset3
154997	4	410037	7	NULL	NULL	0	NULL	thermal midpoint ( T ( m ) ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ferredoxin from the thermophilic archaeon Acidianus ambivalens is a small monomeric seven-iron protein with a thermal midpoint ( T ( m ) ) of 122 degrees C ( pH 7 ) .
	manualset3
154998	5	410037	7	NULL	NULL	0	NULL	122 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ferredoxin from the thermophilic archaeon Acidianus ambivalens is a small monomeric seven-iron protein with a thermal midpoint ( T ( m ) ) of 122 degrees C ( pH 7 ) .
	manualset3
154999	6	410037	7	NULL	NULL	0	NULL	pH 7	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ferredoxin from the thermophilic archaeon Acidianus ambivalens is a small monomeric seven-iron protein with a thermal midpoint ( T ( m ) ) of 122 degrees C ( pH 7 ) .
	manualset3
155000	1	410038	7	NULL	NULL	0	NULL	Clinical analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical analysis of chronic renal function failure accompanied by pulmonary tuberculosis ) .
	manualset3
155001	2	410038	7	NULL	NULL	0	NULL	chronic renal function failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical analysis of chronic renal function failure accompanied by pulmonary tuberculosis ) .
	manualset3
155002	3	410038	7	NULL	NULL	0	NULL	pulmonary tuberculosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical analysis of chronic renal function failure accompanied by pulmonary tuberculosis ) .
	manualset3
155003	1	410039	7	NULL	NULL	0	NULL	ferrocenic bispyrrolo ( 1 , 2-a ) quinoxalines 2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ferrocenic bispyrrolo ( 1 , 2-a ) quinoxalines 2 were prepared by reductive amination of previously described bispyrrolo ( 1 , 2-a ) quinoxalines 9 with ferrocene-carboxaldehyde , by treatment with NaHB ( OAc ) ( 3 ) .
	manualset3
155004	2	410039	7	NULL	NULL	NULL	NULL	reductive amination	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ferrocenic bispyrrolo ( 1 , 2-a ) quinoxalines 2 were prepared by reductive amination of previously described bispyrrolo ( 1 , 2-a ) quinoxalines 9 with ferrocene-carboxaldehyde , by treatment with NaHB ( OAc ) ( 3 ) .
	manualset3
155005	3	410039	7	NULL	NULL	0	NULL	bispyrrolo ( 1 , 2-a ) quinoxalines 9	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ferrocenic bispyrrolo ( 1 , 2-a ) quinoxalines 2 were prepared by reductive amination of previously described bispyrrolo ( 1 , 2-a ) quinoxalines 9 with ferrocene-carboxaldehyde , by treatment with NaHB ( OAc ) ( 3 ) .
	manualset3
155006	4	410039	7	NULL	NULL	0	NULL	ferrocene-carboxaldehyde	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ferrocenic bispyrrolo ( 1 , 2-a ) quinoxalines 2 were prepared by reductive amination of previously described bispyrrolo ( 1 , 2-a ) quinoxalines 9 with ferrocene-carboxaldehyde , by treatment with NaHB ( OAc ) ( 3 ) .
	manualset3
155007	5	410039	7	NULL	NULL	NULL	NULL	NaHB ( OAc )( 3 )	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ferrocenic bispyrrolo ( 1 , 2-a ) quinoxalines 2 were prepared by reductive amination of previously described bispyrrolo ( 1 , 2-a ) quinoxalines 9 with ferrocene-carboxaldehyde , by treatment with NaHB ( OAc ) ( 3 ) .
	manualset3
155008	1	410040	7	NULL	NULL	0	NULL	feruloyl esterase ( StFaeC )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The feruloyl esterase ( StFaeC ) produced by Sporotrichum thermophile transfered the feruloyl group to D : - arabinose using a mixture of n-hexane , t-butanol and water .
	manualset3
155009	2	410040	7	NULL	NULL	0	NULL	Sporotrichum thermophile	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The feruloyl esterase ( StFaeC ) produced by Sporotrichum thermophile transfered the feruloyl group to D : - arabinose using a mixture of n-hexane , t-butanol and water .
	manualset3
155010	3	410040	7	NULL	NULL	0	NULL	feruloyl group	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The feruloyl esterase ( StFaeC ) produced by Sporotrichum thermophile transfered the feruloyl group to D : - arabinose using a mixture of n-hexane , t-butanol and water .
	manualset3
155011	4	410040	7	NULL	NULL	0	NULL	D : - arabinose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The feruloyl esterase ( StFaeC ) produced by Sporotrichum thermophile transfered the feruloyl group to D : - arabinose using a mixture of n-hexane , t-butanol and water .
	manualset3
155012	5	410040	7	NULL	NULL	0	NULL	 n-hexane	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The feruloyl esterase ( StFaeC ) produced by Sporotrichum thermophile transfered the feruloyl group to D : - arabinose using a mixture of n-hexane , t-butanol and water .
	manualset3
155013	6	410040	7	NULL	NULL	0	NULL	t-butanol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The feruloyl esterase ( StFaeC ) produced by Sporotrichum thermophile transfered the feruloyl group to D : - arabinose using a mixture of n-hexane , t-butanol and water .
	manualset3
155014	7	410040	7	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The feruloyl esterase ( StFaeC ) produced by Sporotrichum thermophile transfered the feruloyl group to D : - arabinose using a mixture of n-hexane , t-butanol and water .
	manualset3
157274	8	410040	7	NULL	NULL	NULL	NULL	mixture	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The feruloyl esterase ( StFaeC ) produced by Sporotrichum thermophile transfered the feruloyl group to D : - arabinose using a mixture of n-hexane , t-butanol and water .
	manualset3
155015	1	410041	7	NULL	NULL	0	NULL	field	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The field has , however , seen major technical obstacles to the proficient use of many cytokines .
	manualset3
155016	2	410041	7	NULL	NULL	0	NULL	major technical obstacles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The field has , however , seen major technical obstacles to the proficient use of many cytokines .
	manualset3
155017	3	410041	7	NULL	NULL	0	NULL	cytokines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The field has , however , seen major technical obstacles to the proficient use of many cytokines .
	manualset3
157275	4	410041	7	NULL	NULL	0	NULL	 proficient use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The field has , however , seen major technical obstacles to the proficient use of many cytokines .
	manualset3
155156	1	410042	7	NULL	NULL	0	NULL	fields home	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The fields home ( 98 % ) and family ( 72 % ) presented greater satisfaction for both caregivers and elders .
	manualset3
155157	2	410042	7	NULL	NULL	0	NULL	 98%	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The fields home ( 98 % ) and family ( 72 % ) presented greater satisfaction for both caregivers and elders .
	manualset3
155158	3	410042	7	NULL	NULL	NULL	NULL	 family	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fields home ( 98 % ) and family ( 72 % ) presented greater satisfaction for both caregivers and elders .
	manualset3
155159	4	410042	7	NULL	NULL	0	NULL	72%	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The fields home ( 98 % ) and family ( 72 % ) presented greater satisfaction for both caregivers and elders .
	manualset3
155160	5	410042	7	NULL	NULL	0	NULL	caregivers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The fields home ( 98 % ) and family ( 72 % ) presented greater satisfaction for both caregivers and elders .
	manualset3
155161	6	410042	7	NULL	NULL	0	NULL	elders	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The fields home ( 98 % ) and family ( 72 % ) presented greater satisfaction for both caregivers and elders .
	manualset3
155163	2	410043	7	NULL	NULL	0	NULL	fields of behavioural medicine	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The fields of epidemiology , behavioural medicine and cardiovascular physiology have generated new methodologies for studying the pathophysiology of anger and other behavioural stress states with the goal of developing means to sever the link between the anger and its life-threatening consequences .
	manualset3
155164	3	410043	7	NULL	NULL	0	NULL	fields of cardiovascular physiology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The fields of epidemiology , behavioural medicine and cardiovascular physiology have generated new methodologies for studying the pathophysiology of anger and other behavioural stress states with the goal of developing means to sever the link between the anger and its life-threatening consequences .
	manualset3
155165	4	410043	7	NULL	NULL	0	NULL	new methodologies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The fields of epidemiology , behavioural medicine and cardiovascular physiology have generated new methodologies for studying the pathophysiology of anger and other behavioural stress states with the goal of developing means to sever the link between the anger and its life-threatening consequences .
	manualset3
155166	5	410043	7	NULL	NULL	0	NULL	pathophysiology of anger 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The fields of epidemiology , behavioural medicine and cardiovascular physiology have generated new methodologies for studying the pathophysiology of anger and other behavioural stress states with the goal of developing means to sever the link between the anger and its life-threatening consequences .
	manualset3
155167	6	410043	7	NULL	NULL	0	NULL	behavioural stress states	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The fields of epidemiology , behavioural medicine and cardiovascular physiology have generated new methodologies for studying the pathophysiology of anger and other behavioural stress states with the goal of developing means to sever the link between the anger and its life-threatening consequences .
	manualset3
155168	7	410043	7	NULL	NULL	NULL	NULL	anger	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fields of epidemiology , behavioural medicine and cardiovascular physiology have generated new methodologies for studying the pathophysiology of anger and other behavioural stress states with the goal of developing means to sever the link between the anger and its life-threatening consequences .
	manualset3
155169	8	410043	7	NULL	NULL	0	NULL	life-threatening consequences	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The fields of epidemiology , behavioural medicine and cardiovascular physiology have generated new methodologies for studying the pathophysiology of anger and other behavioural stress states with the goal of developing means to sever the link between the anger and its life-threatening consequences .
	manualset3
157276	9	410043	7	NULL	NULL	0	NULL	fields of epidemiology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The fields of epidemiology , behavioural medicine and cardiovascular physiology have generated new methodologies for studying the pathophysiology of anger and other behavioural stress states with the goal of developing means to sever the link between the anger and its life-threatening consequences .
	manualset3
157278	10	410043	7	NULL	NULL	0	NULL	goal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The fields of epidemiology , behavioural medicine and cardiovascular physiology have generated new methodologies for studying the pathophysiology of anger and other behavioural stress states with the goal of developing means to sever the link between the anger and its life-threatening consequences .
	manualset3
157279	11	410043	7	NULL	NULL	0	NULL	developing means	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The fields of epidemiology , behavioural medicine and cardiovascular physiology have generated new methodologies for studying the pathophysiology of anger and other behavioural stress states with the goal of developing means to sever the link between the anger and its life-threatening consequences .
	manualset3
157280	12	410043	7	NULL	NULL	0	NULL	link	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The fields of epidemiology , behavioural medicine and cardiovascular physiology have generated new methodologies for studying the pathophysiology of anger and other behavioural stress states with the goal of developing means to sever the link between the anger and its life-threatening consequences .
	manualset3
155170	1	410044	7	NULL	NULL	0	NULL	figure	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The figure is significantly different from 50 % , i.e. , two components of equal size can not be assumed .
	manualset3
155171	2	410044	7	NULL	NULL	0	NULL	50 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The figure is significantly different from 50 % , i.e. , two components of equal size can not be assumed .
	manualset3
155172	3	410044	7	NULL	NULL	0	NULL	 two components 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The figure is significantly different from 50 % , i.e. , two components of equal size can not be assumed .
	manualset3
155173	4	410044	7	NULL	NULL	0	NULL	equal size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The figure is significantly different from 50 % , i.e. , two components of equal size can not be assumed .
	manualset3
155218	1	410045	7	NULL	NULL	NULL	NULL	 1710 probands 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The figure of 1710 probands who had survived their first myocardial infarction at an age of 60 to 74 during the time period from 1985 to 1992 was based on the register of acute coronary events with reference to the population of Augsburg , Germany .
	manualset3
155219	2	410045	7	NULL	NULL	0	NULL	myocardial infarction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The figure of 1710 probands who had survived their first myocardial infarction at an age of 60 to 74 during the time period from 1985 to 1992 was based on the register of acute coronary events with reference to the population of Augsburg , Germany .
	manualset3
155220	3	410045	7	NULL	NULL	0	NULL	age of 60 to 74	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The figure of 1710 probands who had survived their first myocardial infarction at an age of 60 to 74 during the time period from 1985 to 1992 was based on the register of acute coronary events with reference to the population of Augsburg , Germany .
	manualset3
155221	4	410045	7	NULL	NULL	0	NULL	time period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The figure of 1710 probands who had survived their first myocardial infarction at an age of 60 to 74 during the time period from 1985 to 1992 was based on the register of acute coronary events with reference to the population of Augsburg , Germany .
	manualset3
155222	5	410045	7	NULL	NULL	0	NULL	1985 to 1992	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The figure of 1710 probands who had survived their first myocardial infarction at an age of 60 to 74 during the time period from 1985 to 1992 was based on the register of acute coronary events with reference to the population of Augsburg , Germany .
	manualset3
155224	6	410045	7	NULL	NULL	0	NULL	acute coronary events	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The figure of 1710 probands who had survived their first myocardial infarction at an age of 60 to 74 during the time period from 1985 to 1992 was based on the register of acute coronary events with reference to the population of Augsburg , Germany .
	manualset3
155226	7	410045	7	NULL	NULL	0	NULL	population 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The figure of 1710 probands who had survived their first myocardial infarction at an age of 60 to 74 during the time period from 1985 to 1992 was based on the register of acute coronary events with reference to the population of Augsburg , Germany .
	manualset3
155229	8	410045	7	NULL	NULL	0	NULL	Augsburg , Germany	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The figure of 1710 probands who had survived their first myocardial infarction at an age of 60 to 74 during the time period from 1985 to 1992 was based on the register of acute coronary events with reference to the population of Augsburg , Germany .
	manualset3
157281	9	410045	7	NULL	NULL	0	NULL	figure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The figure of 1710 probands who had survived their first myocardial infarction at an age of 60 to 74 during the time period from 1985 to 1992 was based on the register of acute coronary events with reference to the population of Augsburg , Germany .
	manualset3
157282	10	410045	7	NULL	NULL	0	NULL	register	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The figure of 1710 probands who had survived their first myocardial infarction at an age of 60 to 74 during the time period from 1985 to 1992 was based on the register of acute coronary events with reference to the population of Augsburg , Germany .
	manualset3
155239	1	410046	7	NULL	NULL	NULL	NULL	filaggrin null genotypes R501X	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The filaggrin null genotypes R501X and 2282del4 seem not to be associated with psoriasis : results from general population study and meta-analysis .
	manualset3
155240	2	410046	7	NULL	NULL	0	NULL	filaggrin null genotypes 2282del4	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The filaggrin null genotypes R501X and 2282del4 seem not to be associated with psoriasis : results from general population study and meta-analysis .
	manualset3
155241	3	410046	7	NULL	NULL	0	NULL	psoriasis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The filaggrin null genotypes R501X and 2282del4 seem not to be associated with psoriasis : results from general population study and meta-analysis .
	manualset3
155246	4	410046	7	NULL	NULL	NULL	NULL	general population study 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The filaggrin null genotypes R501X and 2282del4 seem not to be associated with psoriasis : results from general population study and meta-analysis .
	manualset3
155248	5	410046	7	NULL	NULL	0	NULL	meta-analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The filaggrin null genotypes R501X and 2282del4 seem not to be associated with psoriasis : results from general population study and meta-analysis .
	manualset3
155253	1	410047	7	NULL	NULL	0	NULL	final histological evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The final histological evaluation , however , revealed follicular carcinoma of the thyroid gland .
	manualset3
155255	2	410047	7	NULL	NULL	0	NULL	follicular carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The final histological evaluation , however , revealed follicular carcinoma of the thyroid gland .
	manualset3
155256	3	410047	7	NULL	NULL	0	NULL	 thyroid gland	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The final histological evaluation , however , revealed follicular carcinoma of the thyroid gland .
	manualset3
155257	1	410048	7	NULL	NULL	NULL	NULL	finding of internucleosomal cleavage	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The finding of internucleosomal cleavage of chromatin , perhaps caused by endonuclease activation , has become accepted as a hallmark of this form of cell death .
	manualset3
155258	2	410048	7	NULL	NULL	0	NULL	chromatin	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The finding of internucleosomal cleavage of chromatin , perhaps caused by endonuclease activation , has become accepted as a hallmark of this form of cell death .
	manualset3
155259	3	410048	7	NULL	NULL	0	NULL	endonuclease activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The finding of internucleosomal cleavage of chromatin , perhaps caused by endonuclease activation , has become accepted as a hallmark of this form of cell death .
	manualset3
155260	4	410048	7	NULL	NULL	0	NULL	cell death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The finding of internucleosomal cleavage of chromatin , perhaps caused by endonuclease activation , has become accepted as a hallmark of this form of cell death .
	manualset3
155375	1	410049	7	NULL	NULL	0	NULL	METH	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The finding that METH , but not MDMA , induces microglial effects in the striatum consistent with neurotoxicity might imply different mechanisms of toxic action for these two psychostimulants .
	manualset3
155376	2	410049	7	NULL	NULL	0	NULL	MDMA	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The finding that METH , but not MDMA , induces microglial effects in the striatum consistent with neurotoxicity might imply different mechanisms of toxic action for these two psychostimulants .
	manualset3
155377	3	410049	7	NULL	NULL	0	NULL	microglial effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The finding that METH , but not MDMA , induces microglial effects in the striatum consistent with neurotoxicity might imply different mechanisms of toxic action for these two psychostimulants .
	manualset3
155378	4	410049	7	NULL	NULL	0	NULL	striatum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The finding that METH , but not MDMA , induces microglial effects in the striatum consistent with neurotoxicity might imply different mechanisms of toxic action for these two psychostimulants .
	manualset3
155379	5	410049	7	NULL	NULL	0	NULL	neurotoxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The finding that METH , but not MDMA , induces microglial effects in the striatum consistent with neurotoxicity might imply different mechanisms of toxic action for these two psychostimulants .
	manualset3
155380	6	410049	7	NULL	NULL	NULL	NULL	mechanisms of toxic action	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The finding that METH , but not MDMA , induces microglial effects in the striatum consistent with neurotoxicity might imply different mechanisms of toxic action for these two psychostimulants .
	manualset3
155382	7	410049	7	NULL	NULL	NULL	NULL	psychostimulants	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The finding that METH , but not MDMA , induces microglial effects in the striatum consistent with neurotoxicity might imply different mechanisms of toxic action for these two psychostimulants .
	manualset3
156866	8	410049	7	NULL	NULL	NULL	NULL	The finding	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The finding that METH , but not MDMA , induces microglial effects in the striatum consistent with neurotoxicity might imply different mechanisms of toxic action for these two psychostimulants .
	manualset3
155383	1	410050	7	NULL	NULL	NULL	NULL	proportion	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The finding that the greater proportion of suicide deaths in doctors were by self-poisoning may reflect the fact that doctors have ready access to drugs , and have knowledge of which drugs and doses are likely to cause death .
	manualset3
155384	2	410050	7	NULL	NULL	0	NULL	suicide deaths	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The finding that the greater proportion of suicide deaths in doctors were by self-poisoning may reflect the fact that doctors have ready access to drugs , and have knowledge of which drugs and doses are likely to cause death .
	manualset3
155385	3	410050	7	NULL	NULL	0	NULL	doctors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The finding that the greater proportion of suicide deaths in doctors were by self-poisoning may reflect the fact that doctors have ready access to drugs , and have knowledge of which drugs and doses are likely to cause death .
	manualset3
155386	4	410050	7	NULL	NULL	0	NULL	self-poisoning	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The finding that the greater proportion of suicide deaths in doctors were by self-poisoning may reflect the fact that doctors have ready access to drugs , and have knowledge of which drugs and doses are likely to cause death .
	manualset3
155387	5	410050	7	NULL	NULL	0	NULL	doctors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The finding that the greater proportion of suicide deaths in doctors were by self-poisoning may reflect the fact that doctors have ready access to drugs , and have knowledge of which drugs and doses are likely to cause death .
	manualset3
155388	6	410050	7	NULL	NULL	NULL	NULL	drugs	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The finding that the greater proportion of suicide deaths in doctors were by self-poisoning may reflect the fact that doctors have ready access to drugs , and have knowledge of which drugs and doses are likely to cause death .
	manualset3
155389	7	410050	7	NULL	NULL	NULL	NULL	drugs	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The finding that the greater proportion of suicide deaths in doctors were by self-poisoning may reflect the fact that doctors have ready access to drugs , and have knowledge of which drugs and doses are likely to cause death .
	manualset3
155390	9	410050	7	NULL	NULL	NULL	NULL	death	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The finding that the greater proportion of suicide deaths in doctors were by self-poisoning may reflect the fact that doctors have ready access to drugs , and have knowledge of which drugs and doses are likely to cause death .
	manualset3
156867	10	410050	7	NULL	NULL	NULL	NULL	The finding	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The finding that the greater proportion of suicide deaths in doctors were by self-poisoning may reflect the fact that doctors have ready access to drugs , and have knowledge of which drugs and doses are likely to cause death .
	manualset3
157179	8	410050	7	NULL	NULL	0	NULL	doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The finding that the greater proportion of suicide deaths in doctors were by self-poisoning may reflect the fact that doctors have ready access to drugs , and have knowledge of which drugs and doses are likely to cause death .
	manualset3
157283	11	410050	7	NULL	NULL	0	NULL	access	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The finding that the greater proportion of suicide deaths in doctors were by self-poisoning may reflect the fact that doctors have ready access to drugs , and have knowledge of which drugs and doses are likely to cause death .
	manualset3
157284	12	410050	7	NULL	NULL	0	NULL	knowledge	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The finding that the greater proportion of suicide deaths in doctors were by self-poisoning may reflect the fact that doctors have ready access to drugs , and have knowledge of which drugs and doses are likely to cause death .
	manualset3
155391	1	410051	7	NULL	NULL	NULL	NULL	The findings	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings also reveal a cell death-promoting phenotype for BI-1 that is manifested under low pH conditions .
	manualset3
155392	2	410051	7	NULL	NULL	0	NULL	cell death-promoting phenotype	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings also reveal a cell death-promoting phenotype for BI-1 that is manifested under low pH conditions .
	manualset3
155393	3	410051	7	NULL	NULL	0	NULL	BI-1	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings also reveal a cell death-promoting phenotype for BI-1 that is manifested under low pH conditions .
	manualset3
155394	4	410051	7	NULL	NULL	0	NULL	low pH conditions	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings also reveal a cell death-promoting phenotype for BI-1 that is manifested under low pH conditions .
	manualset3
155395	1	410052	7	NULL	NULL	0	NULL	subsequent decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A subsequent decrease in phosphorylation was attributable to activation of an NMDA/AMPA receptor/Ca2 + / protein phosphatase-2B signaling cascade .
	manualset3
155396	2	410052	7	NULL	NULL	0	NULL	phosphorylation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A subsequent decrease in phosphorylation was attributable to activation of an NMDA/AMPA receptor/Ca2 + / protein phosphatase-2B signaling cascade .
	manualset3
155397	3	410052	7	NULL	NULL	0	NULL	activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A subsequent decrease in phosphorylation was attributable to activation of an NMDA/AMPA receptor/Ca2 + / protein phosphatase-2B signaling cascade .
	manualset3
155398	4	410052	7	NULL	NULL	0	NULL	NMDA/AMPA receptor/Ca2 + / protein phosphatase-2B signaling cascade	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A subsequent decrease in phosphorylation was attributable to activation of an NMDA/AMPA receptor/Ca2 + / protein phosphatase-2B signaling cascade .
	manualset3
155399	1	410053	7	NULL	NULL	NULL	NULL	The findings	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings appear to indicate that after the elimination of major confounding factors , the substantially higher rates of Caesarean section in Newark ( 17.5 % versus 5.8 % ) did not bring about a measurable reduction in the rate of neonatal losses .
	manualset3
155400	2	410053	7	NULL	NULL	0	NULL	elimination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings appear to indicate that after the elimination of major confounding factors , the substantially higher rates of Caesarean section in Newark ( 17.5 % versus 5.8 % ) did not bring about a measurable reduction in the rate of neonatal losses .
	manualset3
155401	3	410053	7	NULL	NULL	0	NULL	major confounding factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings appear to indicate that after the elimination of major confounding factors , the substantially higher rates of Caesarean section in Newark ( 17.5 % versus 5.8 % ) did not bring about a measurable reduction in the rate of neonatal losses .
	manualset3
155402	4	410053	7	NULL	NULL	NULL	NULL	rates of Caesarean section	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings appear to indicate that after the elimination of major confounding factors , the substantially higher rates of Caesarean section in Newark ( 17.5 % versus 5.8 % ) did not bring about a measurable reduction in the rate of neonatal losses .
	manualset3
155403	5	410053	7	NULL	NULL	0	NULL	Newark	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings appear to indicate that after the elimination of major confounding factors , the substantially higher rates of Caesarean section in Newark ( 17.5 % versus 5.8 % ) did not bring about a measurable reduction in the rate of neonatal losses .
	manualset3
155404	6	410053	7	NULL	NULL	0	NULL	17.5 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings appear to indicate that after the elimination of major confounding factors , the substantially higher rates of Caesarean section in Newark ( 17.5 % versus 5.8 % ) did not bring about a measurable reduction in the rate of neonatal losses .
	manualset3
155405	7	410053	7	NULL	NULL	0	NULL	5.8 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings appear to indicate that after the elimination of major confounding factors , the substantially higher rates of Caesarean section in Newark ( 17.5 % versus 5.8 % ) did not bring about a measurable reduction in the rate of neonatal losses .
	manualset3
155406	8	410053	7	NULL	NULL	NULL	NULL	measurable reduction	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings appear to indicate that after the elimination of major confounding factors , the substantially higher rates of Caesarean section in Newark ( 17.5 % versus 5.8 % ) did not bring about a measurable reduction in the rate of neonatal losses .
	manualset3
155407	9	410053	7	NULL	NULL	NULL	NULL	rate of neonatal losses	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings appear to indicate that after the elimination of major confounding factors , the substantially higher rates of Caesarean section in Newark ( 17.5 % versus 5.8 % ) did not bring about a measurable reduction in the rate of neonatal losses .
	manualset3
155408	1	410054	7	NULL	NULL	NULL	NULL	The findings	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings are compared with attitudes reported in the North American literature on sex education .
	manualset3
155409	2	410054	7	NULL	NULL	0	NULL	attitudes	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings are compared with attitudes reported in the North American literature on sex education .
	manualset3
155410	3	410054	7	NULL	NULL	0	NULL	North American literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings are compared with attitudes reported in the North American literature on sex education .
	manualset3
155411	4	410054	7	NULL	NULL	0	NULL	sex education	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings are compared with attitudes reported in the North American literature on sex education .
	manualset3
155414	1	410055	7	NULL	NULL	NULL	NULL	The findings 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings are important to practitioners who strive to provide assistance and interventions for African American women as well as other women of color .
	manualset3
155417	2	410055	7	NULL	NULL	0	NULL	practitioners	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings are important to practitioners who strive to provide assistance and interventions for African American women as well as other women of color .
	manualset3
155418	3	410055	7	NULL	NULL	0	NULL	African American women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings are important to practitioners who strive to provide assistance and interventions for African American women as well as other women of color .
	manualset3
155419	4	410055	7	NULL	NULL	0	NULL	women of color	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings are important to practitioners who strive to provide assistance and interventions for African American women as well as other women of color .
	manualset3
157285	5	410055	7	NULL	NULL	0	NULL	assistance	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings are important to practitioners who strive to provide assistance and interventions for African American women as well as other women of color .
	manualset3
157286	6	410055	7	NULL	NULL	0	NULL	 interventions	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings are important to practitioners who strive to provide assistance and interventions for African American women as well as other women of color .
	manualset3
155420	1	410056	7	NULL	NULL	NULL	NULL	 The findings	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings are interpreted as evidence that enteric botulinum infection occurs in human infants whose intestinal tract has not yet been colonized by bacteria which are indigenous to adults and prevent growth of C. botulinum .
	manualset3
155422	2	410056	7	NULL	NULL	0	NULL	enteric botulinum infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings are interpreted as evidence that enteric botulinum infection occurs in human infants whose intestinal tract has not yet been colonized by bacteria which are indigenous to adults and prevent growth of C. botulinum .
	manualset3
155427	3	410056	7	NULL	NULL	0	NULL	human infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings are interpreted as evidence that enteric botulinum infection occurs in human infants whose intestinal tract has not yet been colonized by bacteria which are indigenous to adults and prevent growth of C. botulinum .
	manualset3
155448	4	410056	7	NULL	NULL	0	NULL	 intestinal tract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings are interpreted as evidence that enteric botulinum infection occurs in human infants whose intestinal tract has not yet been colonized by bacteria which are indigenous to adults and prevent growth of C. botulinum .
	manualset3
155450	5	410056	7	NULL	NULL	NULL	NULL	bacteria	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings are interpreted as evidence that enteric botulinum infection occurs in human infants whose intestinal tract has not yet been colonized by bacteria which are indigenous to adults and prevent growth of C. botulinum .
	manualset3
155451	6	410056	7	NULL	NULL	0	NULL	adults 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings are interpreted as evidence that enteric botulinum infection occurs in human infants whose intestinal tract has not yet been colonized by bacteria which are indigenous to adults and prevent growth of C. botulinum .
	manualset3
155453	7	410056	7	NULL	NULL	NULL	NULL	growth 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings are interpreted as evidence that enteric botulinum infection occurs in human infants whose intestinal tract has not yet been colonized by bacteria which are indigenous to adults and prevent growth of C. botulinum .
	manualset3
156868	8	410056	7	NULL	NULL	0	NULL	C. botulinum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings are interpreted as evidence that enteric botulinum infection occurs in human infants whose intestinal tract has not yet been colonized by bacteria which are indigenous to adults and prevent growth of C. botulinum .
	manualset3
157287	9	410056	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings are interpreted as evidence that enteric botulinum infection occurs in human infants whose intestinal tract has not yet been colonized by bacteria which are indigenous to adults and prevent growth of C. botulinum .
	manualset3
155463	1	410057	7	NULL	NULL	NULL	NULL	 The findings	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings from this study indicate that soft tissue artefact ( STA ) in the mid thoracic region ranges between 14 and 16 mm for 35-degrees of rotation .
	manualset3
155464	2	410057	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings from this study indicate that soft tissue artefact ( STA ) in the mid thoracic region ranges between 14 and 16 mm for 35-degrees of rotation .
	manualset3
155465	3	410057	7	NULL	NULL	0	NULL	soft tissue artefact ( STA ) 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings from this study indicate that soft tissue artefact ( STA ) in the mid thoracic region ranges between 14 and 16 mm for 35-degrees of rotation .
	manualset3
155466	4	410057	7	NULL	NULL	0	NULL	mid thoracic region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings from this study indicate that soft tissue artefact ( STA ) in the mid thoracic region ranges between 14 and 16 mm for 35-degrees of rotation .
	manualset3
155467	5	410057	7	NULL	NULL	0	NULL	14 and 16 mm 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings from this study indicate that soft tissue artefact ( STA ) in the mid thoracic region ranges between 14 and 16 mm for 35-degrees of rotation .
	manualset3
155468	6	410057	7	NULL	NULL	0	NULL	35-degrees of rotation	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings from this study indicate that soft tissue artefact ( STA ) in the mid thoracic region ranges between 14 and 16 mm for 35-degrees of rotation .
	manualset3
155476	1	410058	7	NULL	NULL	NULL	NULL	The findings	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings in the in vitro model system indicate that these oral mucosa equivalents exhibit similarities to the in vivo situation of non-cornified gingiva , thus rendering them a suitable model for the assessment of stages during epithelial reconstruction or in vivo relevant studies on material effects .
	manualset3
155478	2	410058	7	NULL	NULL	0	NULL	in vitro model system	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings in the in vitro model system indicate that these oral mucosa equivalents exhibit similarities to the in vivo situation of non-cornified gingiva , thus rendering them a suitable model for the assessment of stages during epithelial reconstruction or in vivo relevant studies on material effects .
	manualset3
155481	3	410058	7	NULL	NULL	0	NULL	oral mucosa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings in the in vitro model system indicate that these oral mucosa equivalents exhibit similarities to the in vivo situation of non-cornified gingiva , thus rendering them a suitable model for the assessment of stages during epithelial reconstruction or in vivo relevant studies on material effects .
	manualset3
155485	4	410058	7	NULL	NULL	0	NULL	in vivo situation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings in the in vitro model system indicate that these oral mucosa equivalents exhibit similarities to the in vivo situation of non-cornified gingiva , thus rendering them a suitable model for the assessment of stages during epithelial reconstruction or in vivo relevant studies on material effects .
	manualset3
155492	5	410058	7	NULL	NULL	0	NULL	non-cornified gingiva	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings in the in vitro model system indicate that these oral mucosa equivalents exhibit similarities to the in vivo situation of non-cornified gingiva , thus rendering them a suitable model for the assessment of stages during epithelial reconstruction or in vivo relevant studies on material effects .
	manualset3
155494	6	410058	7	NULL	NULL	0	NULL	suitable model 	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings in the in vitro model system indicate that these oral mucosa equivalents exhibit similarities to the in vivo situation of non-cornified gingiva , thus rendering them a suitable model for the assessment of stages during epithelial reconstruction or in vivo relevant studies on material effects .
	manualset3
155496	7	410058	7	NULL	NULL	0	NULL	stages	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings in the in vitro model system indicate that these oral mucosa equivalents exhibit similarities to the in vivo situation of non-cornified gingiva , thus rendering them a suitable model for the assessment of stages during epithelial reconstruction or in vivo relevant studies on material effects .
	manualset3
155499	8	410058	7	NULL	NULL	0	NULL	epithelial reconstruction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings in the in vitro model system indicate that these oral mucosa equivalents exhibit similarities to the in vivo situation of non-cornified gingiva , thus rendering them a suitable model for the assessment of stages during epithelial reconstruction or in vivo relevant studies on material effects .
	manualset3
155507	10	410058	7	NULL	NULL	0	NULL	material effects	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings in the in vitro model system indicate that these oral mucosa equivalents exhibit similarities to the in vivo situation of non-cornified gingiva , thus rendering them a suitable model for the assessment of stages during epithelial reconstruction or in vivo relevant studies on material effects .
	manualset3
157288	11	410058	7	NULL	NULL	0	NULL	assessment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings in the in vitro model system indicate that these oral mucosa equivalents exhibit similarities to the in vivo situation of non-cornified gingiva , thus rendering them a suitable model for the assessment of stages during epithelial reconstruction or in vivo relevant studies on material effects .
	manualset3
157490	12	410058	7	NULL	NULL	0	NULL	similarities	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings in the in vitro model system indicate that these oral mucosa equivalents exhibit similarities to the in vivo situation of non-cornified gingiva , thus rendering them a suitable model for the assessment of stages during epithelial reconstruction or in vivo relevant studies on material effects .
	manualset3
155508	1	410059	7	NULL	NULL	NULL	NULL	The findings	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings indicate that HPV infection may be related to a proportion of head and neck carcinomas but its association is not as clear as that found in cervical cancer .
	manualset3
155509	2	410059	7	NULL	NULL	0	NULL	HPV infection	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings indicate that HPV infection may be related to a proportion of head and neck carcinomas but its association is not as clear as that found in cervical cancer .
	manualset3
155510	3	410059	7	NULL	NULL	NULL	NULL	head and neck carcinomas	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings indicate that HPV infection may be related to a proportion of head and neck carcinomas but its association is not as clear as that found in cervical cancer .
	manualset3
155512	4	410059	7	NULL	NULL	0	NULL	association	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings indicate that HPV infection may be related to a proportion of head and neck carcinomas but its association is not as clear as that found in cervical cancer .
	manualset3
155515	5	410059	7	NULL	NULL	0	NULL	cervical cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings indicate that HPV infection may be related to a proportion of head and neck carcinomas but its association is not as clear as that found in cervical cancer .
	manualset3
157289	6	410059	7	NULL	NULL	0	NULL	proportion	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings indicate that HPV infection may be related to a proportion of head and neck carcinomas but its association is not as clear as that found in cervical cancer .
	manualset3
155518	1	410060	7	NULL	NULL	NULL	NULL	 5 SP animals	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A subset of 5 SP and 5 NSP animals were killed and portions of each cerebral hemisphere , the cerebellum and the brainstem medulla were analyzed for glutamine synthetase ( GS ) .
	manualset3
155519	2	410060	7	NULL	NULL	0	NULL	5 NSP animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A subset of 5 SP and 5 NSP animals were killed and portions of each cerebral hemisphere , the cerebellum and the brainstem medulla were analyzed for glutamine synthetase ( GS ) .
	manualset3
155521	3	410060	7	NULL	NULL	0	NULL	cerebral hemisphere	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A subset of 5 SP and 5 NSP animals were killed and portions of each cerebral hemisphere , the cerebellum and the brainstem medulla were analyzed for glutamine synthetase ( GS ) .
	manualset3
155523	4	410060	7	NULL	NULL	0	NULL	cerebellum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A subset of 5 SP and 5 NSP animals were killed and portions of each cerebral hemisphere , the cerebellum and the brainstem medulla were analyzed for glutamine synthetase ( GS ) .
	manualset3
155525	5	410060	7	NULL	NULL	0	NULL	brainstem medulla	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A subset of 5 SP and 5 NSP animals were killed and portions of each cerebral hemisphere , the cerebellum and the brainstem medulla were analyzed for glutamine synthetase ( GS ) .
	manualset3
155526	6	410060	7	NULL	NULL	0	NULL	glutamine synthetase ( GS )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A subset of 5 SP and 5 NSP animals were killed and portions of each cerebral hemisphere , the cerebellum and the brainstem medulla were analyzed for glutamine synthetase ( GS ) .
	manualset3
157180	7	410060	7	NULL	NULL	NULL	NULL	subset	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A subset of 5 SP and 5 NSP animals were killed and portions of each cerebral hemisphere , the cerebellum and the brainstem medulla were analyzed for glutamine synthetase ( GS ) .
	manualset3
157290	8	410060	7	NULL	NULL	0	NULL	portions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A subset of 5 SP and 5 NSP animals were killed and portions of each cerebral hemisphere , the cerebellum and the brainstem medulla were analyzed for glutamine synthetase ( GS ) .
	manualset3
155527	1	410061	7	NULL	NULL	NULL	NULL	The findings	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings indicate that alterations of the adenomatous polyposis coli and the p53 genes are relatively frequent in sporadic ampullary carcinomas .
	manualset3
155529	2	410061	7	NULL	NULL	0	NULL	adenomatous polyposis coli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings indicate that alterations of the adenomatous polyposis coli and the p53 genes are relatively frequent in sporadic ampullary carcinomas .
	manualset3
155532	3	410061	7	NULL	NULL	0	NULL	 p53 genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings indicate that alterations of the adenomatous polyposis coli and the p53 genes are relatively frequent in sporadic ampullary carcinomas .
	manualset3
155536	4	410061	7	NULL	NULL	0	NULL	sporadic ampullary carcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings indicate that alterations of the adenomatous polyposis coli and the p53 genes are relatively frequent in sporadic ampullary carcinomas .
	manualset3
157291	5	410061	7	NULL	NULL	0	NULL	alterations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings indicate that alterations of the adenomatous polyposis coli and the p53 genes are relatively frequent in sporadic ampullary carcinomas .
	manualset3
155702	1	410062	7	NULL	NULL	NULL	NULL	The findings	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings may be utilized as an assay method for comparative evaluation of specific activation units of the purified basic seminal coagulum proteins or their cleavage products and for quantifying the total basic protein ( pI ) 3.8 ) units in human seminal plasma .
	manualset3
155703	2	410062	7	NULL	NULL	0	NULL	assay method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings may be utilized as an assay method for comparative evaluation of specific activation units of the purified basic seminal coagulum proteins or their cleavage products and for quantifying the total basic protein ( pI ) 3.8 ) units in human seminal plasma .
	manualset3
155704	3	410062	7	NULL	NULL	NULL	NULL	specific activation units	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings may be utilized as an assay method for comparative evaluation of specific activation units of the purified basic seminal coagulum proteins or their cleavage products and for quantifying the total basic protein ( pI ) 3.8 ) units in human seminal plasma .
	manualset3
155705	4	410062	7	NULL	NULL	0	NULL	purified basic seminal coagulum proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings may be utilized as an assay method for comparative evaluation of specific activation units of the purified basic seminal coagulum proteins or their cleavage products and for quantifying the total basic protein ( pI ) 3.8 ) units in human seminal plasma .
	manualset3
155706	5	410062	7	NULL	NULL	NULL	NULL	cleavage products	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings may be utilized as an assay method for comparative evaluation of specific activation units of the purified basic seminal coagulum proteins or their cleavage products and for quantifying the total basic protein ( pI ) 3.8 ) units in human seminal plasma .
	manualset3
155707	6	410062	7	NULL	NULL	0	NULL	 total basic protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings may be utilized as an assay method for comparative evaluation of specific activation units of the purified basic seminal coagulum proteins or their cleavage products and for quantifying the total basic protein ( pI ) 3.8 ) units in human seminal plasma .
	manualset3
155708	7	410062	7	NULL	NULL	0	NULL	( pI ) 3.8 ) units	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings may be utilized as an assay method for comparative evaluation of specific activation units of the purified basic seminal coagulum proteins or their cleavage products and for quantifying the total basic protein ( pI ) 3.8 ) units in human seminal plasma .
	manualset3
155709	8	410062	7	NULL	NULL	0	NULL	human seminal plasma	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings may be utilized as an assay method for comparative evaluation of specific activation units of the purified basic seminal coagulum proteins or their cleavage products and for quantifying the total basic protein ( pI ) 3.8 ) units in human seminal plasma .
	manualset3
156869	9	410062	7	NULL	NULL	0	NULL	comparative evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings may be utilized as an assay method for comparative evaluation of specific activation units of the purified basic seminal coagulum proteins or their cleavage products and for quantifying the total basic protein ( pI ) 3.8 ) units in human seminal plasma .
	manualset3
155710	1	410063	7	NULL	NULL	NULL	NULL	The findings	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings of this study demonstrated that 5-HT2A receptor mRNA was expressed with low to moderate levels in lumbar spinal dorsal horn , NRM , vlPAG and DRN .
	manualset3
155711	2	410063	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings of this study demonstrated that 5-HT2A receptor mRNA was expressed with low to moderate levels in lumbar spinal dorsal horn , NRM , vlPAG and DRN .
	manualset3
155712	3	410063	7	NULL	NULL	0	NULL	5-HT2A receptor mRNA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings of this study demonstrated that 5-HT2A receptor mRNA was expressed with low to moderate levels in lumbar spinal dorsal horn , NRM , vlPAG and DRN .
	manualset3
155713	4	410063	7	NULL	NULL	0	NULL	lumbar spinal dorsal horn	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings of this study demonstrated that 5-HT2A receptor mRNA was expressed with low to moderate levels in lumbar spinal dorsal horn , NRM , vlPAG and DRN .
	manualset3
155764	5	410063	7	NULL	NULL	NULL	NULL	NRM	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings of this study demonstrated that 5-HT2A receptor mRNA was expressed with low to moderate levels in lumbar spinal dorsal horn , NRM , vlPAG and DRN .
	manualset3
155765	6	410063	7	NULL	NULL	0	NULL	vlPAG	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings of this study demonstrated that 5-HT2A receptor mRNA was expressed with low to moderate levels in lumbar spinal dorsal horn , NRM , vlPAG and DRN .
	manualset3
155766	7	410063	7	NULL	NULL	0	NULL	DRN	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings of this study demonstrated that 5-HT2A receptor mRNA was expressed with low to moderate levels in lumbar spinal dorsal horn , NRM , vlPAG and DRN .
	manualset3
157181	8	410063	7	NULL	NULL	NULL	NULL	moderate levels	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings of this study demonstrated that 5-HT2A receptor mRNA was expressed with low to moderate levels in lumbar spinal dorsal horn , NRM , vlPAG and DRN .
	manualset3
155767	1	410064	7	NULL	NULL	NULL	NULL	The findings	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings on social factors are compared and areas for further research are suggested .
	manualset3
155768	2	410064	7	NULL	NULL	0	NULL	social factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings on social factors are compared and areas for further research are suggested .
	manualset3
155769	3	410064	7	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings on social factors are compared and areas for further research are suggested .
	manualset3
157292	4	410064	7	NULL	NULL	0	NULL	areas	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings on social factors are compared and areas for further research are suggested .
	manualset3
155770	1	410065	7	NULL	NULL	NULL	NULL	The findings	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings revealed that human chromosome samples can be stored at -20 degrees C for short periods of time ( approximately several weeks ) , but storage over 3 months compromises chromatin stability .
	manualset3
155771	2	410065	7	NULL	NULL	0	NULL	human chromosome samples	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings revealed that human chromosome samples can be stored at -20 degrees C for short periods of time ( approximately several weeks ) , but storage over 3 months compromises chromatin stability .
	manualset3
155772	3	410065	7	NULL	NULL	0	NULL	-20 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings revealed that human chromosome samples can be stored at -20 degrees C for short periods of time ( approximately several weeks ) , but storage over 3 months compromises chromatin stability .
	manualset3
155773	4	410065	7	NULL	NULL	0	NULL	short periods of time	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings revealed that human chromosome samples can be stored at -20 degrees C for short periods of time ( approximately several weeks ) , but storage over 3 months compromises chromatin stability .
	manualset3
155774	5	410065	7	NULL	NULL	NULL	NULL	several weeks	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings revealed that human chromosome samples can be stored at -20 degrees C for short periods of time ( approximately several weeks ) , but storage over 3 months compromises chromatin stability .
	manualset3
155775	6	410065	7	NULL	NULL	NULL	NULL	storage	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings revealed that human chromosome samples can be stored at -20 degrees C for short periods of time ( approximately several weeks ) , but storage over 3 months compromises chromatin stability .
	manualset3
155776	7	410065	7	NULL	NULL	0	NULL	3 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings revealed that human chromosome samples can be stored at -20 degrees C for short periods of time ( approximately several weeks ) , but storage over 3 months compromises chromatin stability .
	manualset3
155777	8	410065	7	NULL	NULL	0	NULL	chromatin stability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings revealed that human chromosome samples can be stored at -20 degrees C for short periods of time ( approximately several weeks ) , but storage over 3 months compromises chromatin stability .
	manualset3
157293	9	410065	7	NULL	NULL	0	NULL	storage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings revealed that human chromosome samples can be stored at -20 degrees C for short periods of time ( approximately several weeks ) , but storage over 3 months compromises chromatin stability .
	manualset3
155778	1	410066	7	NULL	NULL	NULL	NULL	The findings	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings show that TGF-alpha is , like EGF , a constant component of human tear fluid .
	manualset3
155779	2	410066	7	NULL	NULL	0	NULL	TGF-alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings show that TGF-alpha is , like EGF , a constant component of human tear fluid .
	manualset3
155780	3	410066	7	NULL	NULL	0	NULL	EGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings show that TGF-alpha is , like EGF , a constant component of human tear fluid .
	manualset3
155781	4	410066	7	NULL	NULL	0	NULL	human tear fluid 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings show that TGF-alpha is , like EGF , a constant component of human tear fluid .
	manualset3
157294	5	410066	7	NULL	NULL	0	NULL	component	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings show that TGF-alpha is , like EGF , a constant component of human tear fluid .
	manualset3
155782	1	410067	7	NULL	NULL	NULL	NULL	The findings	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings show that the influential factors can be predicted from the cat owners ' socio-economic status , mainly education and income , as well as gender and age .
	manualset3
155783	2	410067	7	NULL	NULL	0	NULL	influential factors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings show that the influential factors can be predicted from the cat owners ' socio-economic status , mainly education and income , as well as gender and age .
	manualset3
155784	3	410067	7	NULL	NULL	0	NULL	 cat owners	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings show that the influential factors can be predicted from the cat owners ' socio-economic status , mainly education and income , as well as gender and age .
	manualset3
155785	4	410067	7	NULL	NULL	NULL	NULL	socio-economic status	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings show that the influential factors can be predicted from the cat owners ' socio-economic status , mainly education and income , as well as gender and age .
	manualset3
155786	5	410067	7	NULL	NULL	NULL	NULL	education 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings show that the influential factors can be predicted from the cat owners ' socio-economic status , mainly education and income , as well as gender and age .
	manualset3
155787	6	410067	7	NULL	NULL	0	NULL	income	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings show that the influential factors can be predicted from the cat owners ' socio-economic status , mainly education and income , as well as gender and age .
	manualset3
155788	7	410067	7	NULL	NULL	0	NULL	gender	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings show that the influential factors can be predicted from the cat owners ' socio-economic status , mainly education and income , as well as gender and age .
	manualset3
155789	8	410067	7	NULL	NULL	0	NULL	age	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings show that the influential factors can be predicted from the cat owners ' socio-economic status , mainly education and income , as well as gender and age .
	manualset3
155790	1	410068	7	NULL	NULL	NULL	NULL	The findings 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings suggest that , as previously reported for other cytokines , IL-8 is well conserved and deeply involved in immune functions from invertebrates to mammals .
	manualset3
155791	2	410068	7	NULL	NULL	NULL	NULL	cytokines	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings suggest that , as previously reported for other cytokines , IL-8 is well conserved and deeply involved in immune functions from invertebrates to mammals .
	manualset3
155792	3	410068	7	NULL	NULL	NULL	NULL	IL-8	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings suggest that , as previously reported for other cytokines , IL-8 is well conserved and deeply involved in immune functions from invertebrates to mammals .
	manualset3
155793	4	410068	7	NULL	NULL	0	NULL	immune functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings suggest that , as previously reported for other cytokines , IL-8 is well conserved and deeply involved in immune functions from invertebrates to mammals .
	manualset3
155794	5	410068	7	NULL	NULL	0	NULL	 invertebrates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings suggest that , as previously reported for other cytokines , IL-8 is well conserved and deeply involved in immune functions from invertebrates to mammals .
	manualset3
155795	6	410068	7	NULL	NULL	0	NULL	mammals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings suggest that , as previously reported for other cytokines , IL-8 is well conserved and deeply involved in immune functions from invertebrates to mammals .
	manualset3
155797	1	410069	7	NULL	NULL	NULL	NULL	The findings	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings suggest that potentiation of the ASR by disgust and fear depends on the integrity of the anteromedial temporal lobe .
	manualset3
155798	2	410069	7	NULL	NULL	0	NULL	ASR	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings suggest that potentiation of the ASR by disgust and fear depends on the integrity of the anteromedial temporal lobe .
	manualset3
155799	3	410069	7	NULL	NULL	NULL	NULL	disgust	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings suggest that potentiation of the ASR by disgust and fear depends on the integrity of the anteromedial temporal lobe .
	manualset3
155800	4	410069	7	NULL	NULL	NULL	NULL	fear	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings suggest that potentiation of the ASR by disgust and fear depends on the integrity of the anteromedial temporal lobe .
	manualset3
155801	5	410069	7	NULL	NULL	0	NULL	 integrity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings suggest that potentiation of the ASR by disgust and fear depends on the integrity of the anteromedial temporal lobe .
	manualset3
155802	6	410069	7	NULL	NULL	0	NULL	anteromedial temporal lobe	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings suggest that potentiation of the ASR by disgust and fear depends on the integrity of the anteromedial temporal lobe .
	manualset3
157295	7	410069	7	NULL	NULL	0	NULL	potentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings suggest that potentiation of the ASR by disgust and fear depends on the integrity of the anteromedial temporal lobe .
	manualset3
155803	1	410070	7	NULL	NULL	NULL	NULL	 The findings 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings suggest that the antirejection Css threshold for CsA may be at least 75 ng/ml , and the toxicity threshold above 250 ng/ml .
	manualset3
155804	2	410070	7	NULL	NULL	NULL	NULL	antirejection Css threshold	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings suggest that the antirejection Css threshold for CsA may be at least 75 ng/ml , and the toxicity threshold above 250 ng/ml .
	manualset3
155805	3	410070	7	NULL	NULL	0	NULL	CsA	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings suggest that the antirejection Css threshold for CsA may be at least 75 ng/ml , and the toxicity threshold above 250 ng/ml .
	manualset3
155806	4	410070	7	NULL	NULL	0	NULL	75 ng/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings suggest that the antirejection Css threshold for CsA may be at least 75 ng/ml , and the toxicity threshold above 250 ng/ml .
	manualset3
155807	5	410070	7	NULL	NULL	0	NULL	toxicity threshold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings suggest that the antirejection Css threshold for CsA may be at least 75 ng/ml , and the toxicity threshold above 250 ng/ml .
	manualset3
155808	6	410070	7	NULL	NULL	0	NULL	250 ng/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings suggest that the antirejection Css threshold for CsA may be at least 75 ng/ml , and the toxicity threshold above 250 ng/ml .
	manualset3
156062	1	410071	7	NULL	NULL	0	NULL	subset	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A subset of nontypeable Haemophilus influenzae ( NTHI ) biotype IV isolates from the human genital tract or from infected newborn infants forms a cryptic genospecies characterized by , among other features , the presence of peritrichous pili .
	manualset3
156065	2	410071	7	NULL	NULL	NULL	NULL	nontypeable Haemophilus influenzae ( NTHI ) biotype IV isolates	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A subset of nontypeable Haemophilus influenzae ( NTHI ) biotype IV isolates from the human genital tract or from infected newborn infants forms a cryptic genospecies characterized by , among other features , the presence of peritrichous pili .
	manualset3
156073	3	410071	7	NULL	NULL	0	NULL	human genital tract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A subset of nontypeable Haemophilus influenzae ( NTHI ) biotype IV isolates from the human genital tract or from infected newborn infants forms a cryptic genospecies characterized by , among other features , the presence of peritrichous pili .
	manualset3
156074	4	410071	7	NULL	NULL	0	NULL	infected newborn infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A subset of nontypeable Haemophilus influenzae ( NTHI ) biotype IV isolates from the human genital tract or from infected newborn infants forms a cryptic genospecies characterized by , among other features , the presence of peritrichous pili .
	manualset3
156078	5	410071	7	NULL	NULL	0	NULL	cryptic genospecies	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A subset of nontypeable Haemophilus influenzae ( NTHI ) biotype IV isolates from the human genital tract or from infected newborn infants forms a cryptic genospecies characterized by , among other features , the presence of peritrichous pili .
	manualset3
156080	6	410071	7	NULL	NULL	0	NULL	peritrichous pili	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A subset of nontypeable Haemophilus influenzae ( NTHI ) biotype IV isolates from the human genital tract or from infected newborn infants forms a cryptic genospecies characterized by , among other features , the presence of peritrichous pili .
	manualset3
157296	7	410071	7	NULL	NULL	0	NULL	features	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A subset of nontypeable Haemophilus influenzae ( NTHI ) biotype IV isolates from the human genital tract or from infected newborn infants forms a cryptic genospecies characterized by , among other features , the presence of peritrichous pili .
	manualset3
157297	8	410071	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A subset of nontypeable Haemophilus influenzae ( NTHI ) biotype IV isolates from the human genital tract or from infected newborn infants forms a cryptic genospecies characterized by , among other features , the presence of peritrichous pili .
	manualset3
156095	1	410072	7	NULL	NULL	0	NULL	fine structure	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The fine structure of labeled spinothalamic terminals in the central lateral nucleus has been studied in the rat following injection of wheat germ agglutinin-horseradish peroxidase into the spinal cord .
	manualset3
156101	2	410072	7	NULL	NULL	0	NULL	labeled spinothalamic terminals	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The fine structure of labeled spinothalamic terminals in the central lateral nucleus has been studied in the rat following injection of wheat germ agglutinin-horseradish peroxidase into the spinal cord .
	manualset3
156105	3	410072	7	NULL	NULL	0	NULL	central lateral nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The fine structure of labeled spinothalamic terminals in the central lateral nucleus has been studied in the rat following injection of wheat germ agglutinin-horseradish peroxidase into the spinal cord .
	manualset3
156109	4	410072	7	NULL	NULL	0	NULL	rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The fine structure of labeled spinothalamic terminals in the central lateral nucleus has been studied in the rat following injection of wheat germ agglutinin-horseradish peroxidase into the spinal cord .
	manualset3
156113	5	410072	7	NULL	NULL	0	NULL	wheat germ agglutinin-horseradish peroxidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The fine structure of labeled spinothalamic terminals in the central lateral nucleus has been studied in the rat following injection of wheat germ agglutinin-horseradish peroxidase into the spinal cord .
	manualset3
156115	6	410072	7	NULL	NULL	0	NULL	spinal cord 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The fine structure of labeled spinothalamic terminals in the central lateral nucleus has been studied in the rat following injection of wheat germ agglutinin-horseradish peroxidase into the spinal cord .
	manualset3
156871	7	410072	7	NULL	NULL	0	NULL	injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The fine structure of labeled spinothalamic terminals in the central lateral nucleus has been studied in the rat following injection of wheat germ agglutinin-horseradish peroxidase into the spinal cord .
	manualset3
156121	1	410073	7	NULL	NULL	NULL	NULL	finite-difference time-domain method	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The finite-difference time-domain method is first used to model this dual-tuned volume coil and calculate the B ( 1 ) field distributions at two frequencies .
	manualset3
156126	2	410073	7	NULL	NULL	0	NULL	dual-tuned volume coil 	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The finite-difference time-domain method is first used to model this dual-tuned volume coil and calculate the B ( 1 ) field distributions at two frequencies .
	manualset3
156130	3	410073	7	NULL	NULL	NULL	NULL	B ( 1 ) field distributions	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The finite-difference time-domain method is first used to model this dual-tuned volume coil and calculate the B ( 1 ) field distributions at two frequencies .
	manualset3
156142	4	410073	7	NULL	NULL	0	NULL	two frequencies	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The finite-difference time-domain method is first used to model this dual-tuned volume coil and calculate the B ( 1 ) field distributions at two frequencies .
	manualset3
156156	1	410074	7	NULL	NULL	0	NULL	first classifications of Sabouraud	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The first , or parasitic classifications of Sabouraud , rests on the morphology of the dermatophytes on the hair in vivo ( Achorion , Trichophyton endothrix or ectothrix microides and megaspores , Microsporum ) or on the absence of growth on the hair in vivo ( Epidermophyton ) .
	manualset3
156157	2	410074	7	NULL	NULL	0	NULL	parasitic classifications of Sabouraud 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The first , or parasitic classifications of Sabouraud , rests on the morphology of the dermatophytes on the hair in vivo ( Achorion , Trichophyton endothrix or ectothrix microides and megaspores , Microsporum ) or on the absence of growth on the hair in vivo ( Epidermophyton ) .
	manualset3
156158	3	410074	7	NULL	NULL	0	NULL	morphology	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The first , or parasitic classifications of Sabouraud , rests on the morphology of the dermatophytes on the hair in vivo ( Achorion , Trichophyton endothrix or ectothrix microides and megaspores , Microsporum ) or on the absence of growth on the hair in vivo ( Epidermophyton ) .
	manualset3
156159	4	410074	7	NULL	NULL	0	NULL	dermatophytes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The first , or parasitic classifications of Sabouraud , rests on the morphology of the dermatophytes on the hair in vivo ( Achorion , Trichophyton endothrix or ectothrix microides and megaspores , Microsporum ) or on the absence of growth on the hair in vivo ( Epidermophyton ) .
	manualset3
156160	5	410074	7	NULL	NULL	0	NULL	hair	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The first , or parasitic classifications of Sabouraud , rests on the morphology of the dermatophytes on the hair in vivo ( Achorion , Trichophyton endothrix or ectothrix microides and megaspores , Microsporum ) or on the absence of growth on the hair in vivo ( Epidermophyton ) .
	manualset3
156161	6	410074	7	NULL	NULL	0	NULL	in vivo	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The first , or parasitic classifications of Sabouraud , rests on the morphology of the dermatophytes on the hair in vivo ( Achorion , Trichophyton endothrix or ectothrix microides and megaspores , Microsporum ) or on the absence of growth on the hair in vivo ( Epidermophyton ) .
	manualset3
156164	7	410074	7	NULL	NULL	0	NULL	Achorion	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The first , or parasitic classifications of Sabouraud , rests on the morphology of the dermatophytes on the hair in vivo ( Achorion , Trichophyton endothrix or ectothrix microides and megaspores , Microsporum ) or on the absence of growth on the hair in vivo ( Epidermophyton ) .
	manualset3
156178	8	410074	7	NULL	NULL	0	NULL	Trichophyton endothrix	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The first , or parasitic classifications of Sabouraud , rests on the morphology of the dermatophytes on the hair in vivo ( Achorion , Trichophyton endothrix or ectothrix microides and megaspores , Microsporum ) or on the absence of growth on the hair in vivo ( Epidermophyton ) .
	manualset3
156184	9	410074	7	NULL	NULL	0	NULL	ectothrix microides	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The first , or parasitic classifications of Sabouraud , rests on the morphology of the dermatophytes on the hair in vivo ( Achorion , Trichophyton endothrix or ectothrix microides and megaspores , Microsporum ) or on the absence of growth on the hair in vivo ( Epidermophyton ) .
	manualset3
156187	10	410074	7	NULL	NULL	0	NULL	megaspores , Microsporum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The first , or parasitic classifications of Sabouraud , rests on the morphology of the dermatophytes on the hair in vivo ( Achorion , Trichophyton endothrix or ectothrix microides and megaspores , Microsporum ) or on the absence of growth on the hair in vivo ( Epidermophyton ) .
	manualset3
156188	11	410074	7	NULL	NULL	0	NULL	absence of growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The first , or parasitic classifications of Sabouraud , rests on the morphology of the dermatophytes on the hair in vivo ( Achorion , Trichophyton endothrix or ectothrix microides and megaspores , Microsporum ) or on the absence of growth on the hair in vivo ( Epidermophyton ) .
	manualset3
156189	12	410074	7	NULL	NULL	0	NULL	 hair	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The first , or parasitic classifications of Sabouraud , rests on the morphology of the dermatophytes on the hair in vivo ( Achorion , Trichophyton endothrix or ectothrix microides and megaspores , Microsporum ) or on the absence of growth on the hair in vivo ( Epidermophyton ) .
	manualset3
156193	14	410074	7	NULL	NULL	0	NULL	Epidermophyton	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The first , or parasitic classifications of Sabouraud , rests on the morphology of the dermatophytes on the hair in vivo ( Achorion , Trichophyton endothrix or ectothrix microides and megaspores , Microsporum ) or on the absence of growth on the hair in vivo ( Epidermophyton ) .
	manualset3
156203	1	410075	7	NULL	NULL	0	NULL	first approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The first approach is based on liquid-liquid microextraction with dichloromethane , and the second uses solid-phase extraction with C18 .
	manualset3
156204	2	410075	7	NULL	NULL	0	NULL	liquid-liquid microextraction with dichloromethane	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The first approach is based on liquid-liquid microextraction with dichloromethane , and the second uses solid-phase extraction with C18 .
	manualset3
156205	3	410075	7	NULL	NULL	0	NULL	solid-phase extraction with C18	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The first approach is based on liquid-liquid microextraction with dichloromethane , and the second uses solid-phase extraction with C18 .
	manualset3
156218	4	410075	7	NULL	NULL	NULL	NULL	second	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The first approach is based on liquid-liquid microextraction with dichloromethane , and the second uses solid-phase extraction with C18 .
	manualset3
156224	1	410076	7	NULL	NULL	NULL	NULL	first attempts	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The first attempts at measuring the optical properties of X-rays such as refraction , reflection and diffraction are described .
	manualset3
156225	2	410076	7	NULL	NULL	0	NULL	optical properties of X-rays	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The first attempts at measuring the optical properties of X-rays such as refraction , reflection and diffraction are described .
	manualset3
156226	3	410076	7	NULL	NULL	0	NULL	refraction 	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The first attempts at measuring the optical properties of X-rays such as refraction , reflection and diffraction are described .
	manualset3
156227	4	410076	7	NULL	NULL	0	NULL	reflection	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The first attempts at measuring the optical properties of X-rays such as refraction , reflection and diffraction are described .
	manualset3
156228	5	410076	7	NULL	NULL	0	NULL	 diffraction	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The first attempts at measuring the optical properties of X-rays such as refraction , reflection and diffraction are described .
	manualset3
156229	1	410077	7	NULL	NULL	0	NULL	first category 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The first category was `` Pedagogical methods in theory '' with the sub-categories Theory and the application of the course in practice , Knowledge of pedagogy and Information as a professional competence .
	manualset3
156230	2	410077	7	NULL	NULL	0	NULL	Pedagogical methods in theory	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The first category was `` Pedagogical methods in theory '' with the sub-categories Theory and the application of the course in practice , Knowledge of pedagogy and Information as a professional competence .
	manualset3
156231	3	410077	7	NULL	NULL	0	NULL	 sub-categories	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The first category was `` Pedagogical methods in theory '' with the sub-categories Theory and the application of the course in practice , Knowledge of pedagogy and Information as a professional competence .
	manualset3
156232	4	410077	7	NULL	NULL	0	NULL	Theory and the application of the course in practice	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The first category was `` Pedagogical methods in theory '' with the sub-categories Theory and the application of the course in practice , Knowledge of pedagogy and Information as a professional competence .
	manualset3
156233	5	410077	7	NULL	NULL	0	NULL	Knowledge of pedagogy and Information as a professional competence 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The first category was `` Pedagogical methods in theory '' with the sub-categories Theory and the application of the course in practice , Knowledge of pedagogy and Information as a professional competence .
	manualset3
156234	1	410078	7	NULL	NULL	0	NULL	substitution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A substitution of a thymine for cytosine resulting in the replacement of an arginine with cysteine at position 104 of the polypeptide chain was found both by DNA sequencing and restriction fragment length polymorphism analysis .
	manualset3
156236	2	410078	7	NULL	NULL	0	NULL	thymine	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A substitution of a thymine for cytosine resulting in the replacement of an arginine with cysteine at position 104 of the polypeptide chain was found both by DNA sequencing and restriction fragment length polymorphism analysis .
	manualset3
156237	3	410078	7	NULL	NULL	0	NULL	cytosine	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A substitution of a thymine for cytosine resulting in the replacement of an arginine with cysteine at position 104 of the polypeptide chain was found both by DNA sequencing and restriction fragment length polymorphism analysis .
	manualset3
156238	4	410078	7	NULL	NULL	0	NULL	arginine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A substitution of a thymine for cytosine resulting in the replacement of an arginine with cysteine at position 104 of the polypeptide chain was found both by DNA sequencing and restriction fragment length polymorphism analysis .
	manualset3
156239	5	410078	7	NULL	NULL	0	NULL	cysteine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A substitution of a thymine for cytosine resulting in the replacement of an arginine with cysteine at position 104 of the polypeptide chain was found both by DNA sequencing and restriction fragment length polymorphism analysis .
	manualset3
156240	6	410078	7	NULL	NULL	0	NULL	 position 104	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A substitution of a thymine for cytosine resulting in the replacement of an arginine with cysteine at position 104 of the polypeptide chain was found both by DNA sequencing and restriction fragment length polymorphism analysis .
	manualset3
156241	7	410078	7	NULL	NULL	0	NULL	polypeptide chain	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	A substitution of a thymine for cytosine resulting in the replacement of an arginine with cysteine at position 104 of the polypeptide chain was found both by DNA sequencing and restriction fragment length polymorphism analysis .
	manualset3
156242	8	410078	7	NULL	NULL	0	NULL	DNA sequencing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A substitution of a thymine for cytosine resulting in the replacement of an arginine with cysteine at position 104 of the polypeptide chain was found both by DNA sequencing and restriction fragment length polymorphism analysis .
	manualset3
156243	9	410078	7	NULL	NULL	0	NULL	restriction fragment length polymorphism analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A substitution of a thymine for cytosine resulting in the replacement of an arginine with cysteine at position 104 of the polypeptide chain was found both by DNA sequencing and restriction fragment length polymorphism analysis .
	manualset3
157298	10	410078	7	NULL	NULL	0	NULL	replacement	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A substitution of a thymine for cytosine resulting in the replacement of an arginine with cysteine at position 104 of the polypeptide chain was found both by DNA sequencing and restriction fragment length polymorphism analysis .
	manualset3
156244	1	410079	7	NULL	NULL	0	NULL	first derivatives 	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The first derivatives of three spectra revealed that the method could reduce the water disturb on and noise in R ( w ) Vis/NIR spectrum .
	manualset3
156245	2	410079	7	NULL	NULL	0	NULL	three spectra	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The first derivatives of three spectra revealed that the method could reduce the water disturb on and noise in R ( w ) Vis/NIR spectrum .
	manualset3
156246	3	410079	7	NULL	NULL	NULL	NULL	method 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The first derivatives of three spectra revealed that the method could reduce the water disturb on and noise in R ( w ) Vis/NIR spectrum .
	manualset3
156247	4	410079	7	NULL	NULL	0	NULL	water disturb 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The first derivatives of three spectra revealed that the method could reduce the water disturb on and noise in R ( w ) Vis/NIR spectrum .
	manualset3
156248	5	410079	7	NULL	NULL	NULL	NULL	noise in R ( w ) Vis/NIR spectrum	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The first derivatives of three spectra revealed that the method could reduce the water disturb on and noise in R ( w ) Vis/NIR spectrum .
	manualset3
156249	1	410080	7	NULL	NULL	0	NULL	first examples	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The first examples of our new proteins recruit the DNA-binding basic helix region of the leucine zipper protein GCN4 .
	manualset3
156250	2	410080	7	NULL	NULL	0	NULL	new proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The first examples of our new proteins recruit the DNA-binding basic helix region of the leucine zipper protein GCN4 .
	manualset3
156251	3	410080	7	NULL	NULL	0	NULL	DNA-binding basic helix region 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The first examples of our new proteins recruit the DNA-binding basic helix region of the leucine zipper protein GCN4 .
	manualset3
156252	4	410080	7	NULL	NULL	0	NULL	leucine zipper protein GCN4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The first examples of our new proteins recruit the DNA-binding basic helix region of the leucine zipper protein GCN4 .
	manualset3
156253	1	410081	7	NULL	NULL	NULL	NULL	first exon	gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The first exon codes for a signal sequence and for part of the `` pro '' region of the zymogen .
	manualset3
156254	2	410081	7	NULL	NULL	0	NULL	signal sequence	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The first exon codes for a signal sequence and for part of the `` pro '' region of the zymogen .
	manualset3
156255	3	410081	7	NULL	NULL	0	NULL	part of the `` pro '' region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The first exon codes for a signal sequence and for part of the `` pro '' region of the zymogen .
	manualset3
156256	4	410081	7	NULL	NULL	0	NULL	zymogen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The first exon codes for a signal sequence and for part of the `` pro '' region of the zymogen .
	manualset3
156257	1	410082	7	NULL	NULL	0	NULL	first green lineage	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The first green lineage cdc25 dual-specificity phosphatase .
	manualset3
156258	2	410082	7	NULL	NULL	0	NULL	cdc25 dual-specificity phosphatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The first green lineage cdc25 dual-specificity phosphatase .
	manualset3
156259	1	410083	7	NULL	NULL	NULL	NULL	first half	PublicationOrCitation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The first half summarizes the requirements of a measure of pain severity for epidemiological research , describes a number of existing measures of pain severity and discusses the appropriateness of these instruments for measuring chronic pain as part of a postal epidemiological survey .
	manualset3
156260	2	410083	7	NULL	NULL	NULL	NULL	measure of pain severity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The first half summarizes the requirements of a measure of pain severity for epidemiological research , describes a number of existing measures of pain severity and discusses the appropriateness of these instruments for measuring chronic pain as part of a postal epidemiological survey .
	manualset3
156261	3	410083	7	NULL	NULL	0	NULL	epidemiological research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The first half summarizes the requirements of a measure of pain severity for epidemiological research , describes a number of existing measures of pain severity and discusses the appropriateness of these instruments for measuring chronic pain as part of a postal epidemiological survey .
	manualset3
156262	4	410083	7	NULL	NULL	NULL	NULL	instruments	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The first half summarizes the requirements of a measure of pain severity for epidemiological research , describes a number of existing measures of pain severity and discusses the appropriateness of these instruments for measuring chronic pain as part of a postal epidemiological survey .
	manualset3
156263	5	410083	7	NULL	NULL	0	NULL	chronic pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The first half summarizes the requirements of a measure of pain severity for epidemiological research , describes a number of existing measures of pain severity and discusses the appropriateness of these instruments for measuring chronic pain as part of a postal epidemiological survey .
	manualset3
156264	6	410083	7	NULL	NULL	0	NULL	postal epidemiological survey	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The first half summarizes the requirements of a measure of pain severity for epidemiological research , describes a number of existing measures of pain severity and discusses the appropriateness of these instruments for measuring chronic pain as part of a postal epidemiological survey .
	manualset3
156872	7	410083	7	NULL	NULL	NULL	NULL	measures of pain severity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The first half summarizes the requirements of a measure of pain severity for epidemiological research , describes a number of existing measures of pain severity and discusses the appropriateness of these instruments for measuring chronic pain as part of a postal epidemiological survey .
	manualset3
157491	8	410083	7	NULL	NULL	0	NULL	appropriateness	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	The first half summarizes the requirements of a measure of pain severity for epidemiological research , describes a number of existing measures of pain severity and discusses the appropriateness of these instruments for measuring chronic pain as part of a postal epidemiological survey .
	manualset3
156265	1	410084	7	NULL	NULL	0	NULL	first	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The first is an optical system that imposes the phase of an object onto a sinusoidal carrier in the form of a phase modulation .
	manualset3
156266	2	410084	7	NULL	NULL	NULL	NULL	 optical system	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The first is an optical system that imposes the phase of an object onto a sinusoidal carrier in the form of a phase modulation .
	manualset3
156267	3	410084	7	NULL	NULL	0	NULL	phase of an object	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The first is an optical system that imposes the phase of an object onto a sinusoidal carrier in the form of a phase modulation .
	manualset3
156268	4	410084	7	NULL	NULL	0	NULL	sinusoidal carrier	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The first is an optical system that imposes the phase of an object onto a sinusoidal carrier in the form of a phase modulation .
	manualset3
156269	5	410084	7	NULL	NULL	0	NULL	phase modulation	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The first is an optical system that imposes the phase of an object onto a sinusoidal carrier in the form of a phase modulation .
	manualset3
156270	1	410085	7	NULL	NULL	0	NULL	first mass spectrometric fragmentation data	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The first mass spectrometric fragmentation data are reported for galloylquinic acids containing between five and eight gallic acid residues .
	manualset3
156271	2	410085	7	NULL	NULL	0	NULL	galloylquinic acids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The first mass spectrometric fragmentation data are reported for galloylquinic acids containing between five and eight gallic acid residues .
	manualset3
156272	3	410085	7	NULL	NULL	0	NULL	five and eight gallic acid residues	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The first mass spectrometric fragmentation data are reported for galloylquinic acids containing between five and eight gallic acid residues .
	manualset3
156273	1	410086	7	NULL	NULL	0	NULL	first method 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The first method used the differential features of fetal organ development that occur in early and mid pregnancy , based on published tables for beagles .
	manualset3
156274	2	410086	7	NULL	NULL	0	NULL	fetal organ development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The first method used the differential features of fetal organ development that occur in early and mid pregnancy , based on published tables for beagles .
	manualset3
156275	3	410086	7	NULL	NULL	0	NULL	early pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The first method used the differential features of fetal organ development that occur in early and mid pregnancy , based on published tables for beagles .
	manualset3
156276	4	410086	7	NULL	NULL	0	NULL	mid pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The first method used the differential features of fetal organ development that occur in early and mid pregnancy , based on published tables for beagles .
	manualset3
156277	5	410086	7	NULL	NULL	0	NULL	published tables	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The first method used the differential features of fetal organ development that occur in early and mid pregnancy , based on published tables for beagles .
	manualset3
156278	6	410086	7	NULL	NULL	0	NULL	beagles	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The first method used the differential features of fetal organ development that occur in early and mid pregnancy , based on published tables for beagles .
	manualset3
157299	7	410086	7	NULL	NULL	0	NULL	differential features	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The first method used the differential features of fetal organ development that occur in early and mid pregnancy , based on published tables for beagles .
	manualset3
156279	1	410087	7	NULL	NULL	0	NULL	first model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The first model takes eight weeks ; it consists of an initial intraperitoneal injection of N-nitrosodiethylamine , six weeks ' administration of test chemical ( s ) beginning two weeks later , partial hepatectomy at week 3 , and analysis of immunohistochemically identified glutathione S-transferase placental form-positive liver-cell foci .
	manualset3
156280	2	410087	7	NULL	NULL	0	NULL	eight weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The first model takes eight weeks ; it consists of an initial intraperitoneal injection of N-nitrosodiethylamine , six weeks ' administration of test chemical ( s ) beginning two weeks later , partial hepatectomy at week 3 , and analysis of immunohistochemically identified glutathione S-transferase placental form-positive liver-cell foci .
	manualset3
156281	3	410087	7	NULL	NULL	0	NULL	intraperitoneal injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The first model takes eight weeks ; it consists of an initial intraperitoneal injection of N-nitrosodiethylamine , six weeks ' administration of test chemical ( s ) beginning two weeks later , partial hepatectomy at week 3 , and analysis of immunohistochemically identified glutathione S-transferase placental form-positive liver-cell foci .
	manualset3
156282	4	410087	7	NULL	NULL	0	NULL	N-nitrosodiethylamine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The first model takes eight weeks ; it consists of an initial intraperitoneal injection of N-nitrosodiethylamine , six weeks ' administration of test chemical ( s ) beginning two weeks later , partial hepatectomy at week 3 , and analysis of immunohistochemically identified glutathione S-transferase placental form-positive liver-cell foci .
	manualset3
156283	5	410087	7	NULL	NULL	0	NULL	six weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The first model takes eight weeks ; it consists of an initial intraperitoneal injection of N-nitrosodiethylamine , six weeks ' administration of test chemical ( s ) beginning two weeks later , partial hepatectomy at week 3 , and analysis of immunohistochemically identified glutathione S-transferase placental form-positive liver-cell foci .
	manualset3
156284	6	410087	7	NULL	NULL	0	NULL	test chemical ( s )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The first model takes eight weeks ; it consists of an initial intraperitoneal injection of N-nitrosodiethylamine , six weeks ' administration of test chemical ( s ) beginning two weeks later , partial hepatectomy at week 3 , and analysis of immunohistochemically identified glutathione S-transferase placental form-positive liver-cell foci .
	manualset3
156285	7	410087	7	NULL	NULL	0	NULL	two weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The first model takes eight weeks ; it consists of an initial intraperitoneal injection of N-nitrosodiethylamine , six weeks ' administration of test chemical ( s ) beginning two weeks later , partial hepatectomy at week 3 , and analysis of immunohistochemically identified glutathione S-transferase placental form-positive liver-cell foci .
	manualset3
156286	8	410087	7	NULL	NULL	NULL	NULL	partial hepatectomy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The first model takes eight weeks ; it consists of an initial intraperitoneal injection of N-nitrosodiethylamine , six weeks ' administration of test chemical ( s ) beginning two weeks later , partial hepatectomy at week 3 , and analysis of immunohistochemically identified glutathione S-transferase placental form-positive liver-cell foci .
	manualset3
156287	9	410087	7	NULL	NULL	0	NULL	 week 3	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The first model takes eight weeks ; it consists of an initial intraperitoneal injection of N-nitrosodiethylamine , six weeks ' administration of test chemical ( s ) beginning two weeks later , partial hepatectomy at week 3 , and analysis of immunohistochemically identified glutathione S-transferase placental form-positive liver-cell foci .
	manualset3
156288	10	410087	7	NULL	NULL	0	NULL	glutathione S-transferase placental form-positive liver-cell foci	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The first model takes eight weeks ; it consists of an initial intraperitoneal injection of N-nitrosodiethylamine , six weeks ' administration of test chemical ( s ) beginning two weeks later , partial hepatectomy at week 3 , and analysis of immunohistochemically identified glutathione S-transferase placental form-positive liver-cell foci .
	manualset3
156873	11	410087	7	NULL	NULL	0	NULL	administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The first model takes eight weeks ; it consists of an initial intraperitoneal injection of N-nitrosodiethylamine , six weeks ' administration of test chemical ( s ) beginning two weeks later , partial hepatectomy at week 3 , and analysis of immunohistochemically identified glutathione S-transferase placental form-positive liver-cell foci .
	manualset3
157182	12	410087	7	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The first model takes eight weeks ; it consists of an initial intraperitoneal injection of N-nitrosodiethylamine , six weeks ' administration of test chemical ( s ) beginning two weeks later , partial hepatectomy at week 3 , and analysis of immunohistochemically identified glutathione S-transferase placental form-positive liver-cell foci .
	manualset3
156289	1	410088	7	NULL	NULL	0	NULL	first mutation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The first mutation in a multigeneration JME family has been recently found in the alpha1-subunit of the GABAA receptor ( GABRA1 ) , predicting the single amino acid substitution A322D .
	manualset3
156290	2	410088	7	NULL	NULL	0	NULL	multigeneration JME family	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The first mutation in a multigeneration JME family has been recently found in the alpha1-subunit of the GABAA receptor ( GABRA1 ) , predicting the single amino acid substitution A322D .
	manualset3
156291	3	410088	7	NULL	NULL	0	NULL	alpha1-subunit	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The first mutation in a multigeneration JME family has been recently found in the alpha1-subunit of the GABAA receptor ( GABRA1 ) , predicting the single amino acid substitution A322D .
	manualset3
156292	4	410088	7	NULL	NULL	0	NULL	GABAA receptor ( GABRA1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The first mutation in a multigeneration JME family has been recently found in the alpha1-subunit of the GABAA receptor ( GABRA1 ) , predicting the single amino acid substitution A322D .
	manualset3
156293	5	410088	7	NULL	NULL	NULL	NULL	single amino acid substitution A322D	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The first mutation in a multigeneration JME family has been recently found in the alpha1-subunit of the GABAA receptor ( GABRA1 ) , predicting the single amino acid substitution A322D .
	manualset3
156295	1	410089	7	NULL	NULL	0	NULL	first phase	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The first phase is marked by intensification of motor activity because of the direct chelant action on hippocampal synapses .
	manualset3
156296	2	410089	7	NULL	NULL	0	NULL	motor activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The first phase is marked by intensification of motor activity because of the direct chelant action on hippocampal synapses .
	manualset3
156297	3	410089	7	NULL	NULL	0	NULL	direct chelant action	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The first phase is marked by intensification of motor activity because of the direct chelant action on hippocampal synapses .
	manualset3
156298	4	410089	7	NULL	NULL	0	NULL	hippocampal synapses	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The first phase is marked by intensification of motor activity because of the direct chelant action on hippocampal synapses .
	manualset3
157492	5	410089	7	NULL	NULL	0	NULL	intensification	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The first phase is marked by intensification of motor activity because of the direct chelant action on hippocampal synapses .
	manualset3
156299	1	410090	7	NULL	NULL	0	NULL	first phylogenetic analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The first phylogenetic analyses based on cpcBA operon and 16S rRNA gene demonstrated that picocyanobacteria isolates from GML could , with a high bootstrap support , be grouped into five and four clusters , respectively .
	manualset3
156300	2	410090	7	NULL	NULL	0	NULL	cpcBA operon	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The first phylogenetic analyses based on cpcBA operon and 16S rRNA gene demonstrated that picocyanobacteria isolates from GML could , with a high bootstrap support , be grouped into five and four clusters , respectively .
	manualset3
156301	3	410090	7	NULL	NULL	0	NULL	16S rRNA gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The first phylogenetic analyses based on cpcBA operon and 16S rRNA gene demonstrated that picocyanobacteria isolates from GML could , with a high bootstrap support , be grouped into five and four clusters , respectively .
	manualset3
156302	4	410090	7	NULL	NULL	NULL	NULL	picocyanobacteria isolates	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The first phylogenetic analyses based on cpcBA operon and 16S rRNA gene demonstrated that picocyanobacteria isolates from GML could , with a high bootstrap support , be grouped into five and four clusters , respectively .
	manualset3
156303	5	410090	7	NULL	NULL	0	NULL	GML	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The first phylogenetic analyses based on cpcBA operon and 16S rRNA gene demonstrated that picocyanobacteria isolates from GML could , with a high bootstrap support , be grouped into five and four clusters , respectively .
	manualset3
156304	6	410090	7	NULL	NULL	0	NULL	high bootstrap support	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The first phylogenetic analyses based on cpcBA operon and 16S rRNA gene demonstrated that picocyanobacteria isolates from GML could , with a high bootstrap support , be grouped into five and four clusters , respectively .
	manualset3
156305	7	410090	7	NULL	NULL	NULL	NULL	five and four clusters	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The first phylogenetic analyses based on cpcBA operon and 16S rRNA gene demonstrated that picocyanobacteria isolates from GML could , with a high bootstrap support , be grouped into five and four clusters , respectively .
	manualset3
156306	1	410091	7	NULL	NULL	NULL	NULL	first recognition process	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The first recognition process is illustrated by a sarcoma-related ( Src ) protein kinase which catalyzes phosphorylation transfer of a ferrocenoyl-phosphoryl group , from the ferrocene-labeled adenosine triphosphate ( Fc-ATP ) co-substrate , to the surface-bound target peptide and induces a current response .
	manualset3
156307	2	410091	7	NULL	NULL	0	NULL	sarcoma-related ( Src ) protein kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The first recognition process is illustrated by a sarcoma-related ( Src ) protein kinase which catalyzes phosphorylation transfer of a ferrocenoyl-phosphoryl group , from the ferrocene-labeled adenosine triphosphate ( Fc-ATP ) co-substrate , to the surface-bound target peptide and induces a current response .
	manualset3
156308	3	410091	7	NULL	NULL	0	NULL	phosphorylation transfer	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The first recognition process is illustrated by a sarcoma-related ( Src ) protein kinase which catalyzes phosphorylation transfer of a ferrocenoyl-phosphoryl group , from the ferrocene-labeled adenosine triphosphate ( Fc-ATP ) co-substrate , to the surface-bound target peptide and induces a current response .
	manualset3
156309	4	410091	7	NULL	NULL	0	NULL	ferrocenoyl-phosphoryl group	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The first recognition process is illustrated by a sarcoma-related ( Src ) protein kinase which catalyzes phosphorylation transfer of a ferrocenoyl-phosphoryl group , from the ferrocene-labeled adenosine triphosphate ( Fc-ATP ) co-substrate , to the surface-bound target peptide and induces a current response .
	manualset3
156310	5	410091	7	NULL	NULL	0	NULL	ferrocene-labeled adenosine triphosphate ( Fc-ATP ) co-substrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The first recognition process is illustrated by a sarcoma-related ( Src ) protein kinase which catalyzes phosphorylation transfer of a ferrocenoyl-phosphoryl group , from the ferrocene-labeled adenosine triphosphate ( Fc-ATP ) co-substrate , to the surface-bound target peptide and induces a current response .
	manualset3
156311	6	410091	7	NULL	NULL	0	NULL	surface-bound target peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The first recognition process is illustrated by a sarcoma-related ( Src ) protein kinase which catalyzes phosphorylation transfer of a ferrocenoyl-phosphoryl group , from the ferrocene-labeled adenosine triphosphate ( Fc-ATP ) co-substrate , to the surface-bound target peptide and induces a current response .
	manualset3
157300	7	410091	7	NULL	NULL	0	NULL	current response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The first recognition process is illustrated by a sarcoma-related ( Src ) protein kinase which catalyzes phosphorylation transfer of a ferrocenoyl-phosphoryl group , from the ferrocene-labeled adenosine triphosphate ( Fc-ATP ) co-substrate , to the surface-bound target peptide and induces a current response .
	manualset3
156312	1	410092	7	NULL	NULL	NULL	NULL	first relevant part 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The first relevant part of the strategy is the identification of the cellular sequences flanking the WHV integration in order to select one ( or more ) integration-specific primer .
	manualset3
156313	2	410092	7	NULL	NULL	0	NULL	strategy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The first relevant part of the strategy is the identification of the cellular sequences flanking the WHV integration in order to select one ( or more ) integration-specific primer .
	manualset3
156314	3	410092	7	NULL	NULL	0	NULL	cellular sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The first relevant part of the strategy is the identification of the cellular sequences flanking the WHV integration in order to select one ( or more ) integration-specific primer .
	manualset3
156315	4	410092	7	NULL	NULL	0	NULL	WHV integration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The first relevant part of the strategy is the identification of the cellular sequences flanking the WHV integration in order to select one ( or more ) integration-specific primer .
	manualset3
156316	5	410092	7	NULL	NULL	0	NULL	integration-specific primer	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The first relevant part of the strategy is the identification of the cellular sequences flanking the WHV integration in order to select one ( or more ) integration-specific primer .
	manualset3
157183	6	410092	7	NULL	NULL	0	NULL	one ( or more )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The first relevant part of the strategy is the identification of the cellular sequences flanking the WHV integration in order to select one ( or more ) integration-specific primer .
	manualset3
157301	7	410092	7	NULL	NULL	0	NULL	identification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The first relevant part of the strategy is the identification of the cellular sequences flanking the WHV integration in order to select one ( or more ) integration-specific primer .
	manualset3
156317	1	410093	7	NULL	NULL	0	NULL	myometrial invasion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A suggestion of myometrial invasion or metastatic disease is a contraindication to conservative management .
	manualset3
156318	2	410093	7	NULL	NULL	0	NULL	metastatic disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A suggestion of myometrial invasion or metastatic disease is a contraindication to conservative management .
	manualset3
156319	3	410093	7	NULL	NULL	0	NULL	conservative management	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A suggestion of myometrial invasion or metastatic disease is a contraindication to conservative management .
	manualset3
156874	4	410093	7	NULL	NULL	0	NULL	suggestion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A suggestion of myometrial invasion or metastatic disease is a contraindication to conservative management .
	manualset3
157302	5	410093	7	NULL	NULL	0	NULL	contraindication	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A suggestion of myometrial invasion or metastatic disease is a contraindication to conservative management .
	manualset3
156320	1	410094	7	NULL	NULL	0	NULL	 first steep increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The first steep increase in the rate of mineralization of completed enamel matrix occurs after the first transition from smooth ended ameloblasts to ruffle ended ameloblasts .
	manualset3
156321	2	410094	7	NULL	NULL	0	NULL	rate of mineralization	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The first steep increase in the rate of mineralization of completed enamel matrix occurs after the first transition from smooth ended ameloblasts to ruffle ended ameloblasts .
	manualset3
156322	3	410094	7	NULL	NULL	0	NULL	completed enamel matrix	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The first steep increase in the rate of mineralization of completed enamel matrix occurs after the first transition from smooth ended ameloblasts to ruffle ended ameloblasts .
	manualset3
156323	4	410094	7	NULL	NULL	NULL	NULL	first transition	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The first steep increase in the rate of mineralization of completed enamel matrix occurs after the first transition from smooth ended ameloblasts to ruffle ended ameloblasts .
	manualset3
156324	5	410094	7	NULL	NULL	0	NULL	smooth ended ameloblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The first steep increase in the rate of mineralization of completed enamel matrix occurs after the first transition from smooth ended ameloblasts to ruffle ended ameloblasts .
	manualset3
156325	6	410094	7	NULL	NULL	0	NULL	ruffle ended ameloblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The first steep increase in the rate of mineralization of completed enamel matrix occurs after the first transition from smooth ended ameloblasts to ruffle ended ameloblasts .
	manualset3
156326	1	410095	7	NULL	NULL	NULL	NULL	first successful use	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The first successful use of extracorporeal membrane oxygenation ( ECMO ) was 1976 by Bartlett et al. .
	manualset3
156327	2	410095	7	NULL	NULL	0	NULL	extracorporeal membrane oxygenation ( ECMO )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The first successful use of extracorporeal membrane oxygenation ( ECMO ) was 1976 by Bartlett et al. .
	manualset3
156328	3	410095	7	NULL	NULL	0	NULL	1976	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	The first successful use of extracorporeal membrane oxygenation ( ECMO ) was 1976 by Bartlett et al. .
	manualset3
156329	4	410095	7	NULL	NULL	NULL	NULL	Bartlett et al	PublicationOrCitation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The first successful use of extracorporeal membrane oxygenation ( ECMO ) was 1976 by Bartlett et al. .
	manualset3
156330	1	410096	7	NULL	NULL	0	NULL	first system	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The first system `` LDL '' is a low density lipoprotein .
	manualset3
156331	2	410096	7	NULL	NULL	0	NULL	LDL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The first system `` LDL '' is a low density lipoprotein .
	manualset3
156332	3	410096	7	NULL	NULL	0	NULL	low density lipoprotein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The first system `` LDL '' is a low density lipoprotein .
	manualset3
156333	1	410097	7	NULL	NULL	NULL	NULL	first three cases	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The first three cases include a schwannoma , a neurofibroma , and a desmoid tumor of the brachial plexus region .
	manualset3
156334	2	410097	7	NULL	NULL	0	NULL	schwannoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The first three cases include a schwannoma , a neurofibroma , and a desmoid tumor of the brachial plexus region .
	manualset3
156335	3	410097	7	NULL	NULL	0	NULL	neurofibroma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The first three cases include a schwannoma , a neurofibroma , and a desmoid tumor of the brachial plexus region .
	manualset3
156336	4	410097	7	NULL	NULL	0	NULL	desmoid tumor	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The first three cases include a schwannoma , a neurofibroma , and a desmoid tumor of the brachial plexus region .
	manualset3
156337	5	410097	7	NULL	NULL	0	NULL	brachial plexus region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The first three cases include a schwannoma , a neurofibroma , and a desmoid tumor of the brachial plexus region .
	manualset3
156339	2	410098	7	NULL	NULL	NULL	NULL	first two exons of the gene	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The first two exons of the gene , a and b , lie 22 kb downstream of exons c , d , and e , on the same DNA strand .
	manualset3
156340	3	410098	7	NULL	NULL	0	NULL	a and b	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The first two exons of the gene , a and b , lie 22 kb downstream of exons c , d , and e , on the same DNA strand .
	manualset3
156341	4	410098	7	NULL	NULL	0	NULL	22 kb downstream of exons	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The first two exons of the gene , a and b , lie 22 kb downstream of exons c , d , and e , on the same DNA strand .
	manualset3
156342	5	410098	7	NULL	NULL	0	NULL	c , d , and e	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The first two exons of the gene , a and b , lie 22 kb downstream of exons c , d , and e , on the same DNA strand .
	manualset3
156343	6	410098	7	NULL	NULL	0	NULL	DNA strand	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The first two exons of the gene , a and b , lie 22 kb downstream of exons c , d , and e , on the same DNA strand .
	manualset3
156344	1	410099	7	NULL	NULL	NULL	NULL	first	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The first was created of the patients treated due to allergic rhinitis , the second was composed of patients with adenoids , the third one consisted of patients with cleft palate .
	manualset3
156345	2	410099	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The first was created of the patients treated due to allergic rhinitis , the second was composed of patients with adenoids , the third one consisted of patients with cleft palate .
	manualset3
156346	3	410099	7	NULL	NULL	0	NULL	allergic rhinitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The first was created of the patients treated due to allergic rhinitis , the second was composed of patients with adenoids , the third one consisted of patients with cleft palate .
	manualset3
156347	4	410099	7	NULL	NULL	NULL	NULL	adenoids	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The first was created of the patients treated due to allergic rhinitis , the second was composed of patients with adenoids , the third one consisted of patients with cleft palate .
	manualset3
156348	5	410099	7	NULL	NULL	0	NULL	cleft palate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The first was created of the patients treated due to allergic rhinitis , the second was composed of patients with adenoids , the third one consisted of patients with cleft palate .
	manualset3
157184	6	410099	7	NULL	NULL	0	NULL	second	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The first was created of the patients treated due to allergic rhinitis , the second was composed of patients with adenoids , the third one consisted of patients with cleft palate .
	manualset3
157185	7	410099	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The first was created of the patients treated due to allergic rhinitis , the second was composed of patients with adenoids , the third one consisted of patients with cleft palate .
	manualset3
157186	8	410099	7	NULL	NULL	0	NULL	third one	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The first was created of the patients treated due to allergic rhinitis , the second was composed of patients with adenoids , the third one consisted of patients with cleft palate .
	manualset3
157187	9	410099	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The first was created of the patients treated due to allergic rhinitis , the second was composed of patients with adenoids , the third one consisted of patients with cleft palate .
	manualset3
156349	1	410100	7	NULL	NULL	0	NULL	surface-type uniaxial magnetic anisotropy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A surface-type uniaxial magnetic anisotropy with easy axis parallel to the ripples is observed .
	manualset3
156351	2	410100	7	NULL	NULL	0	NULL	ripples	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A surface-type uniaxial magnetic anisotropy with easy axis parallel to the ripples is observed .
	manualset3
157188	3	410100	7	NULL	NULL	NULL	NULL	easy axis	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A surface-type uniaxial magnetic anisotropy with easy axis parallel to the ripples is observed .
	manualset3
156352	1	410101	7	NULL	NULL	0	NULL	 fish 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The fish were fed for 8 weeks with three diets containing different levels of dietary alpha-tocopheryl acetate ( 289 , 553 , 1 069 mg/kg ) .
	manualset3
156353	2	410101	7	NULL	NULL	0	NULL	8 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The fish were fed for 8 weeks with three diets containing different levels of dietary alpha-tocopheryl acetate ( 289 , 553 , 1 069 mg/kg ) .
	manualset3
156354	3	410101	7	NULL	NULL	0	NULL	three diets	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The fish were fed for 8 weeks with three diets containing different levels of dietary alpha-tocopheryl acetate ( 289 , 553 , 1 069 mg/kg ) .
	manualset3
156355	4	410101	7	NULL	NULL	0	NULL	dietary alpha-tocopheryl acetate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The fish were fed for 8 weeks with three diets containing different levels of dietary alpha-tocopheryl acetate ( 289 , 553 , 1 069 mg/kg ) .
	manualset3
156356	5	410101	7	NULL	NULL	NULL	NULL	289 , 553 , 1 069 mg/kg	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fish were fed for 8 weeks with three diets containing different levels of dietary alpha-tocopheryl acetate ( 289 , 553 , 1 069 mg/kg ) .
	manualset3
157303	6	410101	7	NULL	NULL	0	NULL	levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The fish were fed for 8 weeks with three diets containing different levels of dietary alpha-tocopheryl acetate ( 289 , 553 , 1 069 mg/kg ) .
	manualset3
156357	1	410102	7	NULL	NULL	0	NULL	fits	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The fits provide quantitative information on micellar characteristics such as aggregation number , core size , overall size , solvent fraction in the core , and corona thickness .
	manualset3
156358	2	410102	7	NULL	NULL	0	NULL	quantitative information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The fits provide quantitative information on micellar characteristics such as aggregation number , core size , overall size , solvent fraction in the core , and corona thickness .
	manualset3
156359	3	410102	7	NULL	NULL	0	NULL	micellar characteristics	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The fits provide quantitative information on micellar characteristics such as aggregation number , core size , overall size , solvent fraction in the core , and corona thickness .
	manualset3
156360	4	410102	7	NULL	NULL	NULL	NULL	aggregation number	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fits provide quantitative information on micellar characteristics such as aggregation number , core size , overall size , solvent fraction in the core , and corona thickness .
	manualset3
156361	5	410102	7	NULL	NULL	NULL	NULL	core size 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fits provide quantitative information on micellar characteristics such as aggregation number , core size , overall size , solvent fraction in the core , and corona thickness .
	manualset3
156362	6	410102	7	NULL	NULL	NULL	NULL	overall size	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fits provide quantitative information on micellar characteristics such as aggregation number , core size , overall size , solvent fraction in the core , and corona thickness .
	manualset3
156363	7	410102	7	NULL	NULL	0	NULL	solvent fraction in the core	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The fits provide quantitative information on micellar characteristics such as aggregation number , core size , overall size , solvent fraction in the core , and corona thickness .
	manualset3
156364	8	410102	7	NULL	NULL	0	NULL	corona thickness	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The fits provide quantitative information on micellar characteristics such as aggregation number , core size , overall size , solvent fraction in the core , and corona thickness .
	manualset3
156365	1	410103	7	NULL	NULL	NULL	NULL	five best shots	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The five best shots and five worst shots were selected for each shooter on the basis of four shot quality indicators , and pre-shot EEG alpha power for best shots was compared with that of worst shots .
	manualset3
156366	2	410103	7	NULL	NULL	NULL	NULL	five worst shots	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The five best shots and five worst shots were selected for each shooter on the basis of four shot quality indicators , and pre-shot EEG alpha power for best shots was compared with that of worst shots .
	manualset3
156367	3	410103	7	NULL	NULL	NULL	NULL	shooter	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The five best shots and five worst shots were selected for each shooter on the basis of four shot quality indicators , and pre-shot EEG alpha power for best shots was compared with that of worst shots .
	manualset3
156368	4	410103	7	NULL	NULL	NULL	NULL	four shot quality indicators	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The five best shots and five worst shots were selected for each shooter on the basis of four shot quality indicators , and pre-shot EEG alpha power for best shots was compared with that of worst shots .
	manualset3
156369	5	410103	7	NULL	NULL	NULL	NULL	pre-shot EEG alpha power	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The five best shots and five worst shots were selected for each shooter on the basis of four shot quality indicators , and pre-shot EEG alpha power for best shots was compared with that of worst shots .
	manualset3
156370	6	410103	7	NULL	NULL	NULL	NULL	best shots	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The five best shots and five worst shots were selected for each shooter on the basis of four shot quality indicators , and pre-shot EEG alpha power for best shots was compared with that of worst shots .
	manualset3
156371	7	410103	7	NULL	NULL	NULL	NULL	worst shots	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The five best shots and five worst shots were selected for each shooter on the basis of four shot quality indicators , and pre-shot EEG alpha power for best shots was compared with that of worst shots .
	manualset3
156372	1	410104	7	NULL	NULL	NULL	NULL	five complexes	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The five complexes were tested in three different human tumor cell lines for bioactivity as potential anti-tumor agents , showing selective cytotoxicity on TK-10 cell line .
	manualset3
156373	2	410104	7	NULL	NULL	NULL	NULL	three different human tumor cell lines	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The five complexes were tested in three different human tumor cell lines for bioactivity as potential anti-tumor agents , showing selective cytotoxicity on TK-10 cell line .
	manualset3
156374	3	410104	7	NULL	NULL	0	NULL	bioactivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The five complexes were tested in three different human tumor cell lines for bioactivity as potential anti-tumor agents , showing selective cytotoxicity on TK-10 cell line .
	manualset3
156375	4	410104	7	NULL	NULL	0	NULL	potential anti-tumor agents	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The five complexes were tested in three different human tumor cell lines for bioactivity as potential anti-tumor agents , showing selective cytotoxicity on TK-10 cell line .
	manualset3
156376	5	410104	7	NULL	NULL	NULL	NULL	selective cytotoxicity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The five complexes were tested in three different human tumor cell lines for bioactivity as potential anti-tumor agents , showing selective cytotoxicity on TK-10 cell line .
	manualset3
156377	6	410104	7	NULL	NULL	NULL	NULL	TK-10 cell line	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The five complexes were tested in three different human tumor cell lines for bioactivity as potential anti-tumor agents , showing selective cytotoxicity on TK-10 cell line .
	manualset3
156378	1	410105	7	NULL	NULL	0	NULL	fixed-bed results	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The fixed-bed results indicate the high capacity of the activated carbon for the removal of europium and zinc ions .
	manualset3
156379	2	410105	7	NULL	NULL	0	NULL	 high capacity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The fixed-bed results indicate the high capacity of the activated carbon for the removal of europium and zinc ions .
	manualset3
156380	3	410105	7	NULL	NULL	0	NULL	activated carbon	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The fixed-bed results indicate the high capacity of the activated carbon for the removal of europium and zinc ions .
	manualset3
156381	4	410105	7	NULL	NULL	0	NULL	europium ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The fixed-bed results indicate the high capacity of the activated carbon for the removal of europium and zinc ions .
	manualset3
156382	5	410105	7	NULL	NULL	0	NULL	 zinc ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The fixed-bed results indicate the high capacity of the activated carbon for the removal of europium and zinc ions .
	manualset3
156383	1	410106	7	NULL	NULL	0	NULL	flaF mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The flaF and flaG mutations and two newly identified mutations , flbT and flbA ( P.V. Schoenlein and B. Ely , J. Bacteriol .
	manualset3
156384	2	410106	7	NULL	NULL	0	NULL	flaG mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The flaF and flaG mutations and two newly identified mutations , flbT and flbA ( P.V. Schoenlein and B. Ely , J. Bacteriol .
	manualset3
156385	3	410106	7	NULL	NULL	0	NULL	two newly identified mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The flaF and flaG mutations and two newly identified mutations , flbT and flbA ( P.V. Schoenlein and B. Ely , J. Bacteriol .
	manualset3
156386	4	410106	7	NULL	NULL	0	NULL	flbT	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The flaF and flaG mutations and two newly identified mutations , flbT and flbA ( P.V. Schoenlein and B. Ely , J. Bacteriol .
	manualset3
156387	5	410106	7	NULL	NULL	0	NULL	flbA	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The flaF and flaG mutations and two newly identified mutations , flbT and flbA ( P.V. Schoenlein and B. Ely , J. Bacteriol .
	manualset3
156388	6	410106	7	NULL	NULL	0	NULL	P.V. Schoenlein and B. Ely , J. Bacteriol .	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The flaF and flaG mutations and two newly identified mutations , flbT and flbA ( P.V. Schoenlein and B. Ely , J. Bacteriol .
	manualset3
156389	1	410107	7	NULL	NULL	0	NULL	 flagellate	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The flagellate is possibly T. ( Megatrypanum ) freitasi Rego , Magalhes & Siqueira , 1957 , but its final identification is still pending .
	manualset3
156391	2	410107	7	NULL	NULL	0	NULL	T. ( Megatrypanum ) freitasi Rego	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The flagellate is possibly T. ( Megatrypanum ) freitasi Rego , Magalhes & Siqueira , 1957 , but its final identification is still pending .
	manualset3
156392	3	410107	7	NULL	NULL	0	NULL	Magalhes & Siqueira	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The flagellate is possibly T. ( Megatrypanum ) freitasi Rego , Magalhes & Siqueira , 1957 , but its final identification is still pending .
	manualset3
156393	4	410107	7	NULL	NULL	0	NULL	1957	Timepoint												NULL		0	NULL	NULL	NULL	NULL	NULL	The flagellate is possibly T. ( Megatrypanum ) freitasi Rego , Magalhes & Siqueira , 1957 , but its final identification is still pending .
	manualset3
156394	5	410107	7	NULL	NULL	0	NULL	final identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The flagellate is possibly T. ( Megatrypanum ) freitasi Rego , Magalhes & Siqueira , 1957 , but its final identification is still pending .
	manualset3
156395	1	410108	7	NULL	NULL	0	NULL	flavoprotein ALR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The flavoprotein ALR receives two electrons per subunit from Mia40 , which are then donated through one-electron reactions to two cytochrome c molecules , thus mediating a switch from two-electron to one-electron transfer .
	manualset3
156396	2	410108	7	NULL	NULL	0	NULL	two electrons per subunit	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The flavoprotein ALR receives two electrons per subunit from Mia40 , which are then donated through one-electron reactions to two cytochrome c molecules , thus mediating a switch from two-electron to one-electron transfer .
	manualset3
156397	3	410108	7	NULL	NULL	0	NULL	Mia40	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The flavoprotein ALR receives two electrons per subunit from Mia40 , which are then donated through one-electron reactions to two cytochrome c molecules , thus mediating a switch from two-electron to one-electron transfer .
	manualset3
156398	4	410108	7	NULL	NULL	0	NULL	one-electron reactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The flavoprotein ALR receives two electrons per subunit from Mia40 , which are then donated through one-electron reactions to two cytochrome c molecules , thus mediating a switch from two-electron to one-electron transfer .
	manualset3
156399	5	410108	7	NULL	NULL	0	NULL	two cytochrome c molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The flavoprotein ALR receives two electrons per subunit from Mia40 , which are then donated through one-electron reactions to two cytochrome c molecules , thus mediating a switch from two-electron to one-electron transfer .
	manualset3
156400	6	410108	7	NULL	NULL	NULL	NULL	two-electron 	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The flavoprotein ALR receives two electrons per subunit from Mia40 , which are then donated through one-electron reactions to two cytochrome c molecules , thus mediating a switch from two-electron to one-electron transfer .
	manualset3
156401	7	410108	7	NULL	NULL	0	NULL	one-electron transfer	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The flavoprotein ALR receives two electrons per subunit from Mia40 , which are then donated through one-electron reactions to two cytochrome c molecules , thus mediating a switch from two-electron to one-electron transfer .
	manualset3
157304	8	410108	7	NULL	NULL	0	NULL	switch	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The flavoprotein ALR receives two electrons per subunit from Mia40 , which are then donated through one-electron reactions to two cytochrome c molecules , thus mediating a switch from two-electron to one-electron transfer .
	manualset3
156403	1	410109	7	NULL	NULL	NULL	NULL	flexibility of the molecules	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The flexibility of the molecules was studied by molecular mechanics calculations ( MM2 ) and the van der Waals ' ( vdW ) , and water accessible surface areas were calculated and averaged according to a Boltzmann distribution .
	manualset3
156404	2	410109	7	NULL	NULL	NULL	NULL	molecular mechanics calculations ( MM2 )	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The flexibility of the molecules was studied by molecular mechanics calculations ( MM2 ) and the van der Waals ' ( vdW ) , and water accessible surface areas were calculated and averaged according to a Boltzmann distribution .
	manualset3
156405	3	410109	7	NULL	NULL	NULL	NULL	van der Waals ' ( vdW ) 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The flexibility of the molecules was studied by molecular mechanics calculations ( MM2 ) and the van der Waals ' ( vdW ) , and water accessible surface areas were calculated and averaged according to a Boltzmann distribution .
	manualset3
156406	4	410109	7	NULL	NULL	NULL	NULL	water accessible surface areas 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The flexibility of the molecules was studied by molecular mechanics calculations ( MM2 ) and the van der Waals ' ( vdW ) , and water accessible surface areas were calculated and averaged according to a Boltzmann distribution .
	manualset3
156407	5	410109	7	NULL	NULL	NULL	NULL	Boltzmann distribution	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The flexibility of the molecules was studied by molecular mechanics calculations ( MM2 ) and the van der Waals ' ( vdW ) , and water accessible surface areas were calculated and averaged according to a Boltzmann distribution .
	manualset3
156408	1	410110	7	NULL	NULL	0	NULL	flexibility of the new module	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The flexibility of the new module is demonstrated in its capacity to store any type of experiment that either uses or generates specimens or stock organisms .
	manualset3
156409	2	410110	7	NULL	NULL	0	NULL	experiment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The flexibility of the new module is demonstrated in its capacity to store any type of experiment that either uses or generates specimens or stock organisms .
	manualset3
156410	3	410110	7	NULL	NULL	NULL	NULL	specimens 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The flexibility of the new module is demonstrated in its capacity to store any type of experiment that either uses or generates specimens or stock organisms .
	manualset3
156411	4	410110	7	NULL	NULL	0	NULL	stock organisms 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The flexibility of the new module is demonstrated in its capacity to store any type of experiment that either uses or generates specimens or stock organisms .
	manualset3
157189	5	410110	7	NULL	NULL	0	NULL	capacity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The flexibility of the new module is demonstrated in its capacity to store any type of experiment that either uses or generates specimens or stock organisms .
	manualset3
156412	1	410111	7	NULL	NULL	0	NULL	surface coverage of 1.37 amines per nm 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A surface coverage of 1.37 amines per nm ( 2 ) was estimated and indicated that the monolayer was 28 % as dense as a similar monolayer assembled from thiols on gold .
	manualset3
156413	2	410111	7	NULL	NULL	0	NULL	monolayer	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A surface coverage of 1.37 amines per nm ( 2 ) was estimated and indicated that the monolayer was 28 % as dense as a similar monolayer assembled from thiols on gold .
	manualset3
156414	3	410111	7	NULL	NULL	0	NULL	28 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A surface coverage of 1.37 amines per nm ( 2 ) was estimated and indicated that the monolayer was 28 % as dense as a similar monolayer assembled from thiols on gold .
	manualset3
156416	5	410111	7	NULL	NULL	0	NULL	monolayer assembled from thiols on gold	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A surface coverage of 1.37 amines per nm ( 2 ) was estimated and indicated that the monolayer was 28 % as dense as a similar monolayer assembled from thiols on gold .
	manualset3
156417	1	410112	7	NULL	NULL	0	NULL	flow volume per cardiac cycle	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The flow volume per cardiac cycle was not significantly different between the ture ( 23.1 + / - 5.04 ml/cycle ) and false channel ( 27.1 + / - 10.14 ml/cycle ) .
	manualset3
156418	2	410112	7	NULL	NULL	0	NULL	ture ( 23.1 + / - 5.04 ml/cycle ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The flow volume per cardiac cycle was not significantly different between the ture ( 23.1 + / - 5.04 ml/cycle ) and false channel ( 27.1 + / - 10.14 ml/cycle ) .
	manualset3
156419	3	410112	7	NULL	NULL	0	NULL	false channel ( 27.1 + / - 10.14 ml/cycle )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The flow volume per cardiac cycle was not significantly different between the ture ( 23.1 + / - 5.04 ml/cycle ) and false channel ( 27.1 + / - 10.14 ml/cycle ) .
	manualset3
156420	1	410113	7	NULL	NULL	0	NULL	fluorescence anisotropy ( r ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The fluorescence anisotropy ( r ) of diphenylhexatriene ( DPH ) was measured in different preparations ( bovine spinal cord phosphatidylserine liposomes , rat brain microsomes , liposomes made with rat brain microsomal lipid having different phospholipid : cholesterol ratios ) at temperatures ranging from 10 degrees to 55 degrees C. Phosphatidylserine liposomes exhibited an exponential relationship of r versus temperature , whereas the relationship shown by microsomes and liposomes prepared with microsomal lipid extracts was a linear one .
	manualset3
156421	2	410113	7	NULL	NULL	0	NULL	diphenylhexatriene ( DPH ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The fluorescence anisotropy ( r ) of diphenylhexatriene ( DPH ) was measured in different preparations ( bovine spinal cord phosphatidylserine liposomes , rat brain microsomes , liposomes made with rat brain microsomal lipid having different phospholipid : cholesterol ratios ) at temperatures ranging from 10 degrees to 55 degrees C. Phosphatidylserine liposomes exhibited an exponential relationship of r versus temperature , whereas the relationship shown by microsomes and liposomes prepared with microsomal lipid extracts was a linear one .
	manualset3
156422	3	410113	7	NULL	NULL	NULL	NULL	bovine spinal cord phosphatidylserine liposomes 	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fluorescence anisotropy ( r ) of diphenylhexatriene ( DPH ) was measured in different preparations ( bovine spinal cord phosphatidylserine liposomes , rat brain microsomes , liposomes made with rat brain microsomal lipid having different phospholipid : cholesterol ratios ) at temperatures ranging from 10 degrees to 55 degrees C. Phosphatidylserine liposomes exhibited an exponential relationship of r versus temperature , whereas the relationship shown by microsomes and liposomes prepared with microsomal lipid extracts was a linear one .
	manualset3
156423	4	410113	7	NULL	NULL	NULL	NULL	rat brain microsomes	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fluorescence anisotropy ( r ) of diphenylhexatriene ( DPH ) was measured in different preparations ( bovine spinal cord phosphatidylserine liposomes , rat brain microsomes , liposomes made with rat brain microsomal lipid having different phospholipid : cholesterol ratios ) at temperatures ranging from 10 degrees to 55 degrees C. Phosphatidylserine liposomes exhibited an exponential relationship of r versus temperature , whereas the relationship shown by microsomes and liposomes prepared with microsomal lipid extracts was a linear one .
	manualset3
156424	5	410113	7	NULL	NULL	NULL	NULL	liposomes 	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fluorescence anisotropy ( r ) of diphenylhexatriene ( DPH ) was measured in different preparations ( bovine spinal cord phosphatidylserine liposomes , rat brain microsomes , liposomes made with rat brain microsomal lipid having different phospholipid : cholesterol ratios ) at temperatures ranging from 10 degrees to 55 degrees C. Phosphatidylserine liposomes exhibited an exponential relationship of r versus temperature , whereas the relationship shown by microsomes and liposomes prepared with microsomal lipid extracts was a linear one .
	manualset3
156425	6	410113	7	NULL	NULL	0	NULL	 rat brain microsomal lipid	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The fluorescence anisotropy ( r ) of diphenylhexatriene ( DPH ) was measured in different preparations ( bovine spinal cord phosphatidylserine liposomes , rat brain microsomes , liposomes made with rat brain microsomal lipid having different phospholipid : cholesterol ratios ) at temperatures ranging from 10 degrees to 55 degrees C. Phosphatidylserine liposomes exhibited an exponential relationship of r versus temperature , whereas the relationship shown by microsomes and liposomes prepared with microsomal lipid extracts was a linear one .
	manualset3
156426	7	410113	7	NULL	NULL	0	NULL	phospholipid : cholesterol ratios	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The fluorescence anisotropy ( r ) of diphenylhexatriene ( DPH ) was measured in different preparations ( bovine spinal cord phosphatidylserine liposomes , rat brain microsomes , liposomes made with rat brain microsomal lipid having different phospholipid : cholesterol ratios ) at temperatures ranging from 10 degrees to 55 degrees C. Phosphatidylserine liposomes exhibited an exponential relationship of r versus temperature , whereas the relationship shown by microsomes and liposomes prepared with microsomal lipid extracts was a linear one .
	manualset3
156427	8	410113	7	NULL	NULL	NULL	NULL	temperatures	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fluorescence anisotropy ( r ) of diphenylhexatriene ( DPH ) was measured in different preparations ( bovine spinal cord phosphatidylserine liposomes , rat brain microsomes , liposomes made with rat brain microsomal lipid having different phospholipid : cholesterol ratios ) at temperatures ranging from 10 degrees to 55 degrees C. Phosphatidylserine liposomes exhibited an exponential relationship of r versus temperature , whereas the relationship shown by microsomes and liposomes prepared with microsomal lipid extracts was a linear one .
	manualset3
156428	9	410113	7	NULL	NULL	0	NULL	10 degrees to 55 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The fluorescence anisotropy ( r ) of diphenylhexatriene ( DPH ) was measured in different preparations ( bovine spinal cord phosphatidylserine liposomes , rat brain microsomes , liposomes made with rat brain microsomal lipid having different phospholipid : cholesterol ratios ) at temperatures ranging from 10 degrees to 55 degrees C. Phosphatidylserine liposomes exhibited an exponential relationship of r versus temperature , whereas the relationship shown by microsomes and liposomes prepared with microsomal lipid extracts was a linear one .
	manualset3
156429	10	410113	7	NULL	NULL	NULL	NULL	Phosphatidylserine liposomes	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fluorescence anisotropy ( r ) of diphenylhexatriene ( DPH ) was measured in different preparations ( bovine spinal cord phosphatidylserine liposomes , rat brain microsomes , liposomes made with rat brain microsomal lipid having different phospholipid : cholesterol ratios ) at temperatures ranging from 10 degrees to 55 degrees C. Phosphatidylserine liposomes exhibited an exponential relationship of r versus temperature , whereas the relationship shown by microsomes and liposomes prepared with microsomal lipid extracts was a linear one .
	manualset3
156430	11	410113	7	NULL	NULL	0	NULL	exponential relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The fluorescence anisotropy ( r ) of diphenylhexatriene ( DPH ) was measured in different preparations ( bovine spinal cord phosphatidylserine liposomes , rat brain microsomes , liposomes made with rat brain microsomal lipid having different phospholipid : cholesterol ratios ) at temperatures ranging from 10 degrees to 55 degrees C. Phosphatidylserine liposomes exhibited an exponential relationship of r versus temperature , whereas the relationship shown by microsomes and liposomes prepared with microsomal lipid extracts was a linear one .
	manualset3
156431	12	410113	7	NULL	NULL	0	NULL	r versus temperature	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The fluorescence anisotropy ( r ) of diphenylhexatriene ( DPH ) was measured in different preparations ( bovine spinal cord phosphatidylserine liposomes , rat brain microsomes , liposomes made with rat brain microsomal lipid having different phospholipid : cholesterol ratios ) at temperatures ranging from 10 degrees to 55 degrees C. Phosphatidylserine liposomes exhibited an exponential relationship of r versus temperature , whereas the relationship shown by microsomes and liposomes prepared with microsomal lipid extracts was a linear one .
	manualset3
156432	13	410113	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The fluorescence anisotropy ( r ) of diphenylhexatriene ( DPH ) was measured in different preparations ( bovine spinal cord phosphatidylserine liposomes , rat brain microsomes , liposomes made with rat brain microsomal lipid having different phospholipid : cholesterol ratios ) at temperatures ranging from 10 degrees to 55 degrees C. Phosphatidylserine liposomes exhibited an exponential relationship of r versus temperature , whereas the relationship shown by microsomes and liposomes prepared with microsomal lipid extracts was a linear one .
	manualset3
156433	14	410113	7	NULL	NULL	NULL	NULL	microsomes	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fluorescence anisotropy ( r ) of diphenylhexatriene ( DPH ) was measured in different preparations ( bovine spinal cord phosphatidylserine liposomes , rat brain microsomes , liposomes made with rat brain microsomal lipid having different phospholipid : cholesterol ratios ) at temperatures ranging from 10 degrees to 55 degrees C. Phosphatidylserine liposomes exhibited an exponential relationship of r versus temperature , whereas the relationship shown by microsomes and liposomes prepared with microsomal lipid extracts was a linear one .
	manualset3
156434	15	410113	7	NULL	NULL	NULL	NULL	liposomes 	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fluorescence anisotropy ( r ) of diphenylhexatriene ( DPH ) was measured in different preparations ( bovine spinal cord phosphatidylserine liposomes , rat brain microsomes , liposomes made with rat brain microsomal lipid having different phospholipid : cholesterol ratios ) at temperatures ranging from 10 degrees to 55 degrees C. Phosphatidylserine liposomes exhibited an exponential relationship of r versus temperature , whereas the relationship shown by microsomes and liposomes prepared with microsomal lipid extracts was a linear one .
	manualset3
156435	16	410113	7	NULL	NULL	0	NULL	microsomal lipid extracts	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The fluorescence anisotropy ( r ) of diphenylhexatriene ( DPH ) was measured in different preparations ( bovine spinal cord phosphatidylserine liposomes , rat brain microsomes , liposomes made with rat brain microsomal lipid having different phospholipid : cholesterol ratios ) at temperatures ranging from 10 degrees to 55 degrees C. Phosphatidylserine liposomes exhibited an exponential relationship of r versus temperature , whereas the relationship shown by microsomes and liposomes prepared with microsomal lipid extracts was a linear one .
	manualset3
157305	17	410113	7	NULL	NULL	0	NULL	preparations	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The fluorescence anisotropy ( r ) of diphenylhexatriene ( DPH ) was measured in different preparations ( bovine spinal cord phosphatidylserine liposomes , rat brain microsomes , liposomes made with rat brain microsomal lipid having different phospholipid : cholesterol ratios ) at temperatures ranging from 10 degrees to 55 degrees C. Phosphatidylserine liposomes exhibited an exponential relationship of r versus temperature , whereas the relationship shown by microsomes and liposomes prepared with microsomal lipid extracts was a linear one .
	manualset3
156436	1	410114	7	NULL	NULL	NULL	NULL	fluorescence decay I ( t )	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fluorescence decay I ( t ) and time-resolved spectra I ( lambda , t ) of some porphyrins and chlorins in ethanol and phosphate-buffered aqueous solution were investigated with a time-correlated single-photon-counting apparatus with a mode-locked Ar + laser ( 514.5 nm ) as the excitation source .
	manualset3
156437	2	410114	7	NULL	NULL	0	NULL	time-resolved spectra I ( lambda , t ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The fluorescence decay I ( t ) and time-resolved spectra I ( lambda , t ) of some porphyrins and chlorins in ethanol and phosphate-buffered aqueous solution were investigated with a time-correlated single-photon-counting apparatus with a mode-locked Ar + laser ( 514.5 nm ) as the excitation source .
	manualset3
156438	3	410114	7	NULL	NULL	0	NULL	porphyrins	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The fluorescence decay I ( t ) and time-resolved spectra I ( lambda , t ) of some porphyrins and chlorins in ethanol and phosphate-buffered aqueous solution were investigated with a time-correlated single-photon-counting apparatus with a mode-locked Ar + laser ( 514.5 nm ) as the excitation source .
	manualset3
156439	4	410114	7	NULL	NULL	0	NULL	chlorins in ethanol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The fluorescence decay I ( t ) and time-resolved spectra I ( lambda , t ) of some porphyrins and chlorins in ethanol and phosphate-buffered aqueous solution were investigated with a time-correlated single-photon-counting apparatus with a mode-locked Ar + laser ( 514.5 nm ) as the excitation source .
	manualset3
156440	5	410114	7	NULL	NULL	0	NULL	phosphate-buffered aqueous solution 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The fluorescence decay I ( t ) and time-resolved spectra I ( lambda , t ) of some porphyrins and chlorins in ethanol and phosphate-buffered aqueous solution were investigated with a time-correlated single-photon-counting apparatus with a mode-locked Ar + laser ( 514.5 nm ) as the excitation source .
	manualset3
156441	6	410114	7	NULL	NULL	NULL	NULL	time-correlated single-photon-counting apparatus 	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fluorescence decay I ( t ) and time-resolved spectra I ( lambda , t ) of some porphyrins and chlorins in ethanol and phosphate-buffered aqueous solution were investigated with a time-correlated single-photon-counting apparatus with a mode-locked Ar + laser ( 514.5 nm ) as the excitation source .
	manualset3
156442	7	410114	7	NULL	NULL	0	NULL	excitation source	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The fluorescence decay I ( t ) and time-resolved spectra I ( lambda , t ) of some porphyrins and chlorins in ethanol and phosphate-buffered aqueous solution were investigated with a time-correlated single-photon-counting apparatus with a mode-locked Ar + laser ( 514.5 nm ) as the excitation source .
	manualset3
157190	8	410114	7	NULL	NULL	0	NULL	mode-locked Ar + laser ( 514.5 nm )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The fluorescence decay I ( t ) and time-resolved spectra I ( lambda , t ) of some porphyrins and chlorins in ethanol and phosphate-buffered aqueous solution were investigated with a time-correlated single-photon-counting apparatus with a mode-locked Ar + laser ( 514.5 nm ) as the excitation source .
	manualset3
156444	1	410115	7	NULL	NULL	0	NULL	fluorescence intensity	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The fluorescence intensity or its decay time reflects the modification of the DNA double helix .
	manualset3
156445	2	410115	7	NULL	NULL	0	NULL	fluorescence decay time	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The fluorescence intensity or its decay time reflects the modification of the DNA double helix .
	manualset3
156446	3	410115	7	NULL	NULL	0	NULL	DNA double helix	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The fluorescence intensity or its decay time reflects the modification of the DNA double helix .
	manualset3
156875	4	410115	7	NULL	NULL	0	NULL	modification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The fluorescence intensity or its decay time reflects the modification of the DNA double helix .
	manualset3
156448	1	410116	7	NULL	NULL	0	NULL	fluorescence 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The fluorescence of acrylodan-labeled rod indicated that although the S2 intermediate is unfolded , it is not in a random-coil conformation .
	manualset3
156449	2	410116	7	NULL	NULL	0	NULL	acrylodan-labeled rod	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The fluorescence of acrylodan-labeled rod indicated that although the S2 intermediate is unfolded , it is not in a random-coil conformation .
	manualset3
156450	3	410116	7	NULL	NULL	0	NULL	S2 intermediate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The fluorescence of acrylodan-labeled rod indicated that although the S2 intermediate is unfolded , it is not in a random-coil conformation .
	manualset3
156451	4	410116	7	NULL	NULL	0	NULL	random-coil conformation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The fluorescence of acrylodan-labeled rod indicated that although the S2 intermediate is unfolded , it is not in a random-coil conformation .
	manualset3
156452	1	410117	7	NULL	NULL	0	NULL	flux at 50 keV	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The flux at 50 keV was approximately 2x10 ( 6 ) photons/mm2/s with a rotating anode tungsten x-ray tube operating at 120 kVp and 100 mA .
	manualset3
156453	2	410117	7	NULL	NULL	0	NULL	 2x10 ( 6 ) photons/mm2/s with a rotating anode tungsten x-ray tube	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The flux at 50 keV was approximately 2x10 ( 6 ) photons/mm2/s with a rotating anode tungsten x-ray tube operating at 120 kVp and 100 mA .
	manualset3
156454	3	410117	7	NULL	NULL	0	NULL	120 kVp	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The flux at 50 keV was approximately 2x10 ( 6 ) photons/mm2/s with a rotating anode tungsten x-ray tube operating at 120 kVp and 100 mA .
	manualset3
156455	4	410117	7	NULL	NULL	0	NULL	100 mA	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The flux at 50 keV was approximately 2x10 ( 6 ) photons/mm2/s with a rotating anode tungsten x-ray tube operating at 120 kVp and 100 mA .
	manualset3
156456	1	410118	7	NULL	NULL	0	NULL	flux 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The flux is inhibited by fusicoccin .
	manualset3
156457	2	410118	7	NULL	NULL	0	NULL	fusicoccin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The flux is inhibited by fusicoccin .
	manualset3
156458	1	410119	7	NULL	NULL	0	NULL	focal module	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The focal module is composed of a diaphragmed small telescope used as `` field lens , '' a small cophased diverging Fresnel zone lens that cancels the dispersion , and a detector .
	manualset3
156459	2	410119	7	NULL	NULL	NULL	NULL	diaphragmed small telescope	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The focal module is composed of a diaphragmed small telescope used as `` field lens , '' a small cophased diverging Fresnel zone lens that cancels the dispersion , and a detector .
	manualset3
156460	3	410119	7	NULL	NULL	0	NULL	field lens	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The focal module is composed of a diaphragmed small telescope used as `` field lens , '' a small cophased diverging Fresnel zone lens that cancels the dispersion , and a detector .
	manualset3
156461	4	410119	7	NULL	NULL	0	NULL	small cophased diverging Fresnel zone lens 	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The focal module is composed of a diaphragmed small telescope used as `` field lens , '' a small cophased diverging Fresnel zone lens that cancels the dispersion , and a detector .
	manualset3
156462	5	410119	7	NULL	NULL	0	NULL	dispersion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The focal module is composed of a diaphragmed small telescope used as `` field lens , '' a small cophased diverging Fresnel zone lens that cancels the dispersion , and a detector .
	manualset3
156463	6	410119	7	NULL	NULL	0	NULL	detector	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The focal module is composed of a diaphragmed small telescope used as `` field lens , '' a small cophased diverging Fresnel zone lens that cancels the dispersion , and a detector .
	manualset3
156464	1	410120	7	NULL	NULL	0	NULL	Clinical analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical analysis of seven acute phosphine poisoning ) .
	manualset3
156465	2	410120	7	NULL	NULL	NULL	NULL	seven acute phosphine poisoning 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Clinical analysis of seven acute phosphine poisoning ) .
	manualset3
156466	1	410121	7	NULL	NULL	0	NULL	surface	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A surface that is required for rapid formation of preinitiation complexes ( PICs ) was identified on the N-terminal domain ( NTD ) of the RNA Pol II general transcription factor TFIIA .
	manualset3
156467	2	410121	7	NULL	NULL	NULL	NULL	preinitiation complexes ( PICs )	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A surface that is required for rapid formation of preinitiation complexes ( PICs ) was identified on the N-terminal domain ( NTD ) of the RNA Pol II general transcription factor TFIIA .
	manualset3
156468	3	410121	7	NULL	NULL	0	NULL	N-terminal domain ( NTD )	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A surface that is required for rapid formation of preinitiation complexes ( PICs ) was identified on the N-terminal domain ( NTD ) of the RNA Pol II general transcription factor TFIIA .
	manualset3
156469	4	410121	7	NULL	NULL	0	NULL	RNA Pol II general transcription factor TFIIA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A surface that is required for rapid formation of preinitiation complexes ( PICs ) was identified on the N-terminal domain ( NTD ) of the RNA Pol II general transcription factor TFIIA .
	manualset3
157191	5	410121	7	NULL	NULL	0	NULL	rapid formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A surface that is required for rapid formation of preinitiation complexes ( PICs ) was identified on the N-terminal domain ( NTD ) of the RNA Pol II general transcription factor TFIIA .
	manualset3
156470	1	410122	7	NULL	NULL	0	NULL	focus	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The focus in welfarism may be on utility while that of the decision maker 's approach may be considered to be on health .
	manualset3
156471	2	410122	7	NULL	NULL	0	NULL	welfarism	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The focus in welfarism may be on utility while that of the decision maker 's approach may be considered to be on health .
	manualset3
156472	3	410122	7	NULL	NULL	0	NULL	decision maker 's approach	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The focus in welfarism may be on utility while that of the decision maker 's approach may be considered to be on health .
	manualset3
156473	4	410122	7	NULL	NULL	0	NULL	health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The focus in welfarism may be on utility while that of the decision maker 's approach may be considered to be on health .
	manualset3
157306	5	410122	7	NULL	NULL	0	NULL	utility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The focus in welfarism may be on utility while that of the decision maker 's approach may be considered to be on health .
	manualset3
156474	1	410123	7	NULL	NULL	0	NULL	focus of attention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The focus of attention in this article is on interprofessional relationships , on the roles played by the different professional organizations in the fields of physical education and medicine , the local and national governments , and the judicial system , and on the social , political , and cultural circumstances under which developments in the field of mechanotherapy took place .
	manualset3
156476	2	410123	7	NULL	NULL	0	NULL	 article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The focus of attention in this article is on interprofessional relationships , on the roles played by the different professional organizations in the fields of physical education and medicine , the local and national governments , and the judicial system , and on the social , political , and cultural circumstances under which developments in the field of mechanotherapy took place .
	manualset3
156477	3	410123	7	NULL	NULL	0	NULL	interprofessional relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The focus of attention in this article is on interprofessional relationships , on the roles played by the different professional organizations in the fields of physical education and medicine , the local and national governments , and the judicial system , and on the social , political , and cultural circumstances under which developments in the field of mechanotherapy took place .
	manualset3
156478	4	410123	7	NULL	NULL	0	NULL	professional organizations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The focus of attention in this article is on interprofessional relationships , on the roles played by the different professional organizations in the fields of physical education and medicine , the local and national governments , and the judicial system , and on the social , political , and cultural circumstances under which developments in the field of mechanotherapy took place .
	manualset3
156479	5	410123	7	NULL	NULL	0	NULL	physical education	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The focus of attention in this article is on interprofessional relationships , on the roles played by the different professional organizations in the fields of physical education and medicine , the local and national governments , and the judicial system , and on the social , political , and cultural circumstances under which developments in the field of mechanotherapy took place .
	manualset3
156480	6	410123	7	NULL	NULL	0	NULL	medicine	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The focus of attention in this article is on interprofessional relationships , on the roles played by the different professional organizations in the fields of physical education and medicine , the local and national governments , and the judicial system , and on the social , political , and cultural circumstances under which developments in the field of mechanotherapy took place .
	manualset3
156481	7	410123	7	NULL	NULL	0	NULL	local government	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The focus of attention in this article is on interprofessional relationships , on the roles played by the different professional organizations in the fields of physical education and medicine , the local and national governments , and the judicial system , and on the social , political , and cultural circumstances under which developments in the field of mechanotherapy took place .
	manualset3
156482	8	410123	7	NULL	NULL	0	NULL	national governments	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The focus of attention in this article is on interprofessional relationships , on the roles played by the different professional organizations in the fields of physical education and medicine , the local and national governments , and the judicial system , and on the social , political , and cultural circumstances under which developments in the field of mechanotherapy took place .
	manualset3
156483	9	410123	7	NULL	NULL	0	NULL	mechanotherapy	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The focus of attention in this article is on interprofessional relationships , on the roles played by the different professional organizations in the fields of physical education and medicine , the local and national governments , and the judicial system , and on the social , political , and cultural circumstances under which developments in the field of mechanotherapy took place .
	manualset3
156876	10	410123	7	NULL	NULL	0	NULL	judicial system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The focus of attention in this article is on interprofessional relationships , on the roles played by the different professional organizations in the fields of physical education and medicine , the local and national governments , and the judicial system , and on the social , political , and cultural circumstances under which developments in the field of mechanotherapy took place .
	manualset3
156877	11	410123	7	NULL	NULL	0	NULL	social circumstances	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The focus of attention in this article is on interprofessional relationships , on the roles played by the different professional organizations in the fields of physical education and medicine , the local and national governments , and the judicial system , and on the social , political , and cultural circumstances under which developments in the field of mechanotherapy took place .
	manualset3
156878	12	410123	7	NULL	NULL	0	NULL	political circumstances	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The focus of attention in this article is on interprofessional relationships , on the roles played by the different professional organizations in the fields of physical education and medicine , the local and national governments , and the judicial system , and on the social , political , and cultural circumstances under which developments in the field of mechanotherapy took place .
	manualset3
156879	13	410123	7	NULL	NULL	0	NULL	cultural circumstances	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The focus of attention in this article is on interprofessional relationships , on the roles played by the different professional organizations in the fields of physical education and medicine , the local and national governments , and the judicial system , and on the social , political , and cultural circumstances under which developments in the field of mechanotherapy took place .
	manualset3
157307	14	410123	7	NULL	NULL	0	NULL	developments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The focus of attention in this article is on interprofessional relationships , on the roles played by the different professional organizations in the fields of physical education and medicine , the local and national governments , and the judicial system , and on the social , political , and cultural circumstances under which developments in the field of mechanotherapy took place .
	manualset3
156484	1	410124	7	NULL	NULL	0	NULL	fold	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The fold was originally classified as `` BtrG-like , '' a small family that only includes structures of hypothetical proteins from Mus musculus , Escherichia coli , Pyrococcus horikoshii , and Arabidopsis thaliana .
	manualset3
156485	2	410124	7	NULL	NULL	0	NULL	`` BtrG-like , '' a small family	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The fold was originally classified as `` BtrG-like , '' a small family that only includes structures of hypothetical proteins from Mus musculus , Escherichia coli , Pyrococcus horikoshii , and Arabidopsis thaliana .
	manualset3
156486	3	410124	7	NULL	NULL	0	NULL	hypothetical proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The fold was originally classified as `` BtrG-like , '' a small family that only includes structures of hypothetical proteins from Mus musculus , Escherichia coli , Pyrococcus horikoshii , and Arabidopsis thaliana .
	manualset3
156487	4	410124	7	NULL	NULL	0	NULL	Mus musculus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The fold was originally classified as `` BtrG-like , '' a small family that only includes structures of hypothetical proteins from Mus musculus , Escherichia coli , Pyrococcus horikoshii , and Arabidopsis thaliana .
	manualset3
156488	5	410124	7	NULL	NULL	0	NULL	Escherichia coli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The fold was originally classified as `` BtrG-like , '' a small family that only includes structures of hypothetical proteins from Mus musculus , Escherichia coli , Pyrococcus horikoshii , and Arabidopsis thaliana .
	manualset3
156489	6	410124	7	NULL	NULL	0	NULL	Pyrococcus horikoshii	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The fold was originally classified as `` BtrG-like , '' a small family that only includes structures of hypothetical proteins from Mus musculus , Escherichia coli , Pyrococcus horikoshii , and Arabidopsis thaliana .
	manualset3
156490	7	410124	7	NULL	NULL	0	NULL	Arabidopsis thaliana	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The fold was originally classified as `` BtrG-like , '' a small family that only includes structures of hypothetical proteins from Mus musculus , Escherichia coli , Pyrococcus horikoshii , and Arabidopsis thaliana .
	manualset3
157308	8	410124	7	NULL	NULL	0	NULL	structures	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The fold was originally classified as `` BtrG-like , '' a small family that only includes structures of hypothetical proteins from Mus musculus , Escherichia coli , Pyrococcus horikoshii , and Arabidopsis thaliana .
	manualset3
156491	1	410125	7	NULL	NULL	0	NULL	folding pathway	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The folding pathway of a fast-folding immunoglobulin domain revealed by single-molecule mechanical experiments .
	manualset3
156492	2	410125	7	NULL	NULL	0	NULL	fast-folding immunoglobulin domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The folding pathway of a fast-folding immunoglobulin domain revealed by single-molecule mechanical experiments .
	manualset3
156493	3	410125	7	NULL	NULL	0	NULL	single-molecule mechanical experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The folding pathway of a fast-folding immunoglobulin domain revealed by single-molecule mechanical experiments .
	manualset3
156494	1	410126	7	NULL	NULL	0	NULL	follow-up	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The follow-up was between 5 and 44 years , with a mean of 15 years .
	manualset3
156495	2	410126	7	NULL	NULL	0	NULL	5 and 44 years	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	The follow-up was between 5 and 44 years , with a mean of 15 years .
	manualset3
156496	3	410126	7	NULL	NULL	0	NULL	15 years	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	The follow-up was between 5 and 44 years , with a mean of 15 years .
	manualset3
157309	4	410126	7	NULL	NULL	0	NULL	mean	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The follow-up was between 5 and 44 years , with a mean of 15 years .
	manualset3
156497	1	410127	7	NULL	NULL	0	NULL	SCC	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The following SCC were evaluated in vitro and in vivo : fibrous ground ( FG ) , fibrous composted ( FC ) , NOJAX ground ( NG ) , and NOJAX composted ( NC ) .
	manualset3
156500	4	410127	7	NULL	NULL	0	NULL	fibrous ground ( FG )	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The following SCC were evaluated in vitro and in vivo : fibrous ground ( FG ) , fibrous composted ( FC ) , NOJAX ground ( NG ) , and NOJAX composted ( NC ) .
	manualset3
156501	5	410127	7	NULL	NULL	0	NULL	fibrous composted ( FC )	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The following SCC were evaluated in vitro and in vivo : fibrous ground ( FG ) , fibrous composted ( FC ) , NOJAX ground ( NG ) , and NOJAX composted ( NC ) .
	manualset3
156502	6	410127	7	NULL	NULL	0	NULL	NOJAX ground ( NG )	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The following SCC were evaluated in vitro and in vivo : fibrous ground ( FG ) , fibrous composted ( FC ) , NOJAX ground ( NG ) , and NOJAX composted ( NC ) .
	manualset3
156503	7	410127	7	NULL	NULL	0	NULL	NOJAX composted ( NC )	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The following SCC were evaluated in vitro and in vivo : fibrous ground ( FG ) , fibrous composted ( FC ) , NOJAX ground ( NG ) , and NOJAX composted ( NC ) .
	manualset3
156504	1	410128	7	NULL	NULL	NULL	NULL	abnormalities 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The following abnormalities were observed in our AIDP patients : absent H reflex in 90.7 % , conduction block in the Erb-to-axilla segment in 78.6 % , motor conduction velocity suggestive of demyelination in the Erb-to-axilla segment in 45.2 % , prolonged F wave latency in 65.2 % -73.8 % of patients but only 20.0 % -37.0 % with prolonged F wave latency suggestive of demyelination , and reduced or absent sensory nerve action potential in 62 % of patients .
	manualset3
156505	2	410128	7	NULL	NULL	0	NULL	AIDP patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The following abnormalities were observed in our AIDP patients : absent H reflex in 90.7 % , conduction block in the Erb-to-axilla segment in 78.6 % , motor conduction velocity suggestive of demyelination in the Erb-to-axilla segment in 45.2 % , prolonged F wave latency in 65.2 % -73.8 % of patients but only 20.0 % -37.0 % with prolonged F wave latency suggestive of demyelination , and reduced or absent sensory nerve action potential in 62 % of patients .
	manualset3
156506	3	410128	7	NULL	NULL	0	NULL	absent H reflex in 90.7 %	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The following abnormalities were observed in our AIDP patients : absent H reflex in 90.7 % , conduction block in the Erb-to-axilla segment in 78.6 % , motor conduction velocity suggestive of demyelination in the Erb-to-axilla segment in 45.2 % , prolonged F wave latency in 65.2 % -73.8 % of patients but only 20.0 % -37.0 % with prolonged F wave latency suggestive of demyelination , and reduced or absent sensory nerve action potential in 62 % of patients .
	manualset3
156507	4	410128	7	NULL	NULL	0	NULL	conduction block in the Erb-to-axilla segment in 78.6 % 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The following abnormalities were observed in our AIDP patients : absent H reflex in 90.7 % , conduction block in the Erb-to-axilla segment in 78.6 % , motor conduction velocity suggestive of demyelination in the Erb-to-axilla segment in 45.2 % , prolonged F wave latency in 65.2 % -73.8 % of patients but only 20.0 % -37.0 % with prolonged F wave latency suggestive of demyelination , and reduced or absent sensory nerve action potential in 62 % of patients .
	manualset3
156508	5	410128	7	NULL	NULL	0	NULL	demyelination in the Erb-to-axilla segment in 45.2 %	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The following abnormalities were observed in our AIDP patients : absent H reflex in 90.7 % , conduction block in the Erb-to-axilla segment in 78.6 % , motor conduction velocity suggestive of demyelination in the Erb-to-axilla segment in 45.2 % , prolonged F wave latency in 65.2 % -73.8 % of patients but only 20.0 % -37.0 % with prolonged F wave latency suggestive of demyelination , and reduced or absent sensory nerve action potential in 62 % of patients .
	manualset3
156509	6	410128	7	NULL	NULL	0	NULL	prolonged F wave latency in 65.2 % -73.8 % of patients	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The following abnormalities were observed in our AIDP patients : absent H reflex in 90.7 % , conduction block in the Erb-to-axilla segment in 78.6 % , motor conduction velocity suggestive of demyelination in the Erb-to-axilla segment in 45.2 % , prolonged F wave latency in 65.2 % -73.8 % of patients but only 20.0 % -37.0 % with prolonged F wave latency suggestive of demyelination , and reduced or absent sensory nerve action potential in 62 % of patients .
	manualset3
156510	7	410128	7	NULL	NULL	0	NULL	20.0 % -37.0 % with prolonged F wave latency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The following abnormalities were observed in our AIDP patients : absent H reflex in 90.7 % , conduction block in the Erb-to-axilla segment in 78.6 % , motor conduction velocity suggestive of demyelination in the Erb-to-axilla segment in 45.2 % , prolonged F wave latency in 65.2 % -73.8 % of patients but only 20.0 % -37.0 % with prolonged F wave latency suggestive of demyelination , and reduced or absent sensory nerve action potential in 62 % of patients .
	manualset3
156511	8	410128	7	NULL	NULL	0	NULL	demyelination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The following abnormalities were observed in our AIDP patients : absent H reflex in 90.7 % , conduction block in the Erb-to-axilla segment in 78.6 % , motor conduction velocity suggestive of demyelination in the Erb-to-axilla segment in 45.2 % , prolonged F wave latency in 65.2 % -73.8 % of patients but only 20.0 % -37.0 % with prolonged F wave latency suggestive of demyelination , and reduced or absent sensory nerve action potential in 62 % of patients .
	manualset3
156512	9	410128	7	NULL	NULL	0	NULL	reduced or absent sensory nerve action potential	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The following abnormalities were observed in our AIDP patients : absent H reflex in 90.7 % , conduction block in the Erb-to-axilla segment in 78.6 % , motor conduction velocity suggestive of demyelination in the Erb-to-axilla segment in 45.2 % , prolonged F wave latency in 65.2 % -73.8 % of patients but only 20.0 % -37.0 % with prolonged F wave latency suggestive of demyelination , and reduced or absent sensory nerve action potential in 62 % of patients .
	manualset3
156513	10	410128	7	NULL	NULL	0	NULL	62 % of patients	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The following abnormalities were observed in our AIDP patients : absent H reflex in 90.7 % , conduction block in the Erb-to-axilla segment in 78.6 % , motor conduction velocity suggestive of demyelination in the Erb-to-axilla segment in 45.2 % , prolonged F wave latency in 65.2 % -73.8 % of patients but only 20.0 % -37.0 % with prolonged F wave latency suggestive of demyelination , and reduced or absent sensory nerve action potential in 62 % of patients .
	manualset3
157192	11	410128	7	NULL	NULL	0	NULL	motor conduction velocity	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The following abnormalities were observed in our AIDP patients : absent H reflex in 90.7 % , conduction block in the Erb-to-axilla segment in 78.6 % , motor conduction velocity suggestive of demyelination in the Erb-to-axilla segment in 45.2 % , prolonged F wave latency in 65.2 % -73.8 % of patients but only 20.0 % -37.0 % with prolonged F wave latency suggestive of demyelination , and reduced or absent sensory nerve action potential in 62 % of patients .
	manualset3
156514	1	410129	7	NULL	NULL	0	NULL	factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The following factors are considered to be ARF-provoking : postaggressive circulation centralization , predominant administration of crystalloid plasma substitutes , persistence of hypoproteinemia in the earliest postoperative period , as well as extended lymph dissection involving cardiopulmonary plexus located in the area of bifurcation .
	manualset3
156516	3	410129	7	NULL	NULL	0	NULL	postaggressive circulation centralization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The following factors are considered to be ARF-provoking : postaggressive circulation centralization , predominant administration of crystalloid plasma substitutes , persistence of hypoproteinemia in the earliest postoperative period , as well as extended lymph dissection involving cardiopulmonary plexus located in the area of bifurcation .
	manualset3
156517	4	410129	7	NULL	NULL	0	NULL	crystalloid plasma substitutes	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The following factors are considered to be ARF-provoking : postaggressive circulation centralization , predominant administration of crystalloid plasma substitutes , persistence of hypoproteinemia in the earliest postoperative period , as well as extended lymph dissection involving cardiopulmonary plexus located in the area of bifurcation .
	manualset3
156518	5	410129	7	NULL	NULL	0	NULL	hypoproteinemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The following factors are considered to be ARF-provoking : postaggressive circulation centralization , predominant administration of crystalloid plasma substitutes , persistence of hypoproteinemia in the earliest postoperative period , as well as extended lymph dissection involving cardiopulmonary plexus located in the area of bifurcation .
	manualset3
156519	6	410129	7	NULL	NULL	0	NULL	earliest postoperative period	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The following factors are considered to be ARF-provoking : postaggressive circulation centralization , predominant administration of crystalloid plasma substitutes , persistence of hypoproteinemia in the earliest postoperative period , as well as extended lymph dissection involving cardiopulmonary plexus located in the area of bifurcation .
	manualset3
156520	7	410129	7	NULL	NULL	0	NULL	extended lymph dissection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The following factors are considered to be ARF-provoking : postaggressive circulation centralization , predominant administration of crystalloid plasma substitutes , persistence of hypoproteinemia in the earliest postoperative period , as well as extended lymph dissection involving cardiopulmonary plexus located in the area of bifurcation .
	manualset3
156521	8	410129	7	NULL	NULL	0	NULL	cardiopulmonary plexus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The following factors are considered to be ARF-provoking : postaggressive circulation centralization , predominant administration of crystalloid plasma substitutes , persistence of hypoproteinemia in the earliest postoperative period , as well as extended lymph dissection involving cardiopulmonary plexus located in the area of bifurcation .
	manualset3
156522	9	410129	7	NULL	NULL	0	NULL	area of bifurcation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The following factors are considered to be ARF-provoking : postaggressive circulation centralization , predominant administration of crystalloid plasma substitutes , persistence of hypoproteinemia in the earliest postoperative period , as well as extended lymph dissection involving cardiopulmonary plexus located in the area of bifurcation .
	manualset3
156523	1	410130	7	NULL	NULL	0	NULL	information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The following information was extracted and collated : patient demographics , type and indication of CAM products , system-organ class affected , seriousness of the adverse event , route of administration , hospitalization status , outcome of adverse event , concomitant use of conventional medicine , adulterant testing and profession of the reporter .
	manualset3
156524	2	410130	7	NULL	NULL	0	NULL	patient demographics	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The following information was extracted and collated : patient demographics , type and indication of CAM products , system-organ class affected , seriousness of the adverse event , route of administration , hospitalization status , outcome of adverse event , concomitant use of conventional medicine , adulterant testing and profession of the reporter .
	manualset3
156525	3	410130	7	NULL	NULL	0	NULL	CAM products	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The following information was extracted and collated : patient demographics , type and indication of CAM products , system-organ class affected , seriousness of the adverse event , route of administration , hospitalization status , outcome of adverse event , concomitant use of conventional medicine , adulterant testing and profession of the reporter .
	manualset3
156526	4	410130	7	NULL	NULL	0	NULL	system-organ class affected	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The following information was extracted and collated : patient demographics , type and indication of CAM products , system-organ class affected , seriousness of the adverse event , route of administration , hospitalization status , outcome of adverse event , concomitant use of conventional medicine , adulterant testing and profession of the reporter .
	manualset3
156527	5	410130	7	NULL	NULL	0	NULL	adverse event	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The following information was extracted and collated : patient demographics , type and indication of CAM products , system-organ class affected , seriousness of the adverse event , route of administration , hospitalization status , outcome of adverse event , concomitant use of conventional medicine , adulterant testing and profession of the reporter .
	manualset3
156528	6	410130	7	NULL	NULL	0	NULL	route of administration 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The following information was extracted and collated : patient demographics , type and indication of CAM products , system-organ class affected , seriousness of the adverse event , route of administration , hospitalization status , outcome of adverse event , concomitant use of conventional medicine , adulterant testing and profession of the reporter .
	manualset3
156529	7	410130	7	NULL	NULL	0	NULL	hospitalization status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The following information was extracted and collated : patient demographics , type and indication of CAM products , system-organ class affected , seriousness of the adverse event , route of administration , hospitalization status , outcome of adverse event , concomitant use of conventional medicine , adulterant testing and profession of the reporter .
	manualset3
156530	8	410130	7	NULL	NULL	0	NULL	outcome of adverse event	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The following information was extracted and collated : patient demographics , type and indication of CAM products , system-organ class affected , seriousness of the adverse event , route of administration , hospitalization status , outcome of adverse event , concomitant use of conventional medicine , adulterant testing and profession of the reporter .
	manualset3
156531	9	410130	7	NULL	NULL	0	NULL	conventional medicine	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The following information was extracted and collated : patient demographics , type and indication of CAM products , system-organ class affected , seriousness of the adverse event , route of administration , hospitalization status , outcome of adverse event , concomitant use of conventional medicine , adulterant testing and profession of the reporter .
	manualset3
156532	10	410130	7	NULL	NULL	NULL	NULL	adulterant testing	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The following information was extracted and collated : patient demographics , type and indication of CAM products , system-organ class affected , seriousness of the adverse event , route of administration , hospitalization status , outcome of adverse event , concomitant use of conventional medicine , adulterant testing and profession of the reporter .
	manualset3
156533	11	410130	7	NULL	NULL	NULL	NULL	profession of the reporter	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The following information was extracted and collated : patient demographics , type and indication of CAM products , system-organ class affected , seriousness of the adverse event , route of administration , hospitalization status , outcome of adverse event , concomitant use of conventional medicine , adulterant testing and profession of the reporter .
	manualset3
156535	1	410131	7	NULL	NULL	0	NULL	survey findings	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The following is a summary of the survey findings : The incidence of propoxyphene-associated deaths reached a peak in 1977 , then declined by 22.2 % from 1977 to 1978 and by 33.3 % from 1978 to 1979 , and by a further 10-18 % since then .
	manualset3
156536	2	410131	7	NULL	NULL	0	NULL	 incidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The following is a summary of the survey findings : The incidence of propoxyphene-associated deaths reached a peak in 1977 , then declined by 22.2 % from 1977 to 1978 and by 33.3 % from 1978 to 1979 , and by a further 10-18 % since then .
	manualset3
156537	3	410131	7	NULL	NULL	0	NULL	propoxyphene-associated deaths	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The following is a summary of the survey findings : The incidence of propoxyphene-associated deaths reached a peak in 1977 , then declined by 22.2 % from 1977 to 1978 and by 33.3 % from 1978 to 1979 , and by a further 10-18 % since then .
	manualset3
156538	4	410131	7	NULL	NULL	0	NULL	1977	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	The following is a summary of the survey findings : The incidence of propoxyphene-associated deaths reached a peak in 1977 , then declined by 22.2 % from 1977 to 1978 and by 33.3 % from 1978 to 1979 , and by a further 10-18 % since then .
	manualset3
156539	5	410131	7	NULL	NULL	0	NULL	22.2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The following is a summary of the survey findings : The incidence of propoxyphene-associated deaths reached a peak in 1977 , then declined by 22.2 % from 1977 to 1978 and by 33.3 % from 1978 to 1979 , and by a further 10-18 % since then .
	manualset3
156540	6	410131	7	NULL	NULL	NULL	NULL	1977 to 1978	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The following is a summary of the survey findings : The incidence of propoxyphene-associated deaths reached a peak in 1977 , then declined by 22.2 % from 1977 to 1978 and by 33.3 % from 1978 to 1979 , and by a further 10-18 % since then .
	manualset3
156541	7	410131	7	NULL	NULL	0	NULL	33.3 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The following is a summary of the survey findings : The incidence of propoxyphene-associated deaths reached a peak in 1977 , then declined by 22.2 % from 1977 to 1978 and by 33.3 % from 1978 to 1979 , and by a further 10-18 % since then .
	manualset3
156542	8	410131	7	NULL	NULL	NULL	NULL	1978 to 1979	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The following is a summary of the survey findings : The incidence of propoxyphene-associated deaths reached a peak in 1977 , then declined by 22.2 % from 1977 to 1978 and by 33.3 % from 1978 to 1979 , and by a further 10-18 % since then .
	manualset3
156543	9	410131	7	NULL	NULL	0	NULL	10-18 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The following is a summary of the survey findings : The incidence of propoxyphene-associated deaths reached a peak in 1977 , then declined by 22.2 % from 1977 to 1978 and by 33.3 % from 1978 to 1979 , and by a further 10-18 % since then .
	manualset3
157310	10	410131	7	NULL	NULL	0	NULL	summary	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The following is a summary of the survey findings : The incidence of propoxyphene-associated deaths reached a peak in 1977 , then declined by 22.2 % from 1977 to 1978 and by 33.3 % from 1978 to 1979 , and by a further 10-18 % since then .
	manualset3
156544	1	410132	7	NULL	NULL	0	NULL	 survey interview 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey interview was used to collect data on abused women recruited from the Kaohsiung area in southern Taiwan .
	manualset3
156545	2	410132	7	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey interview was used to collect data on abused women recruited from the Kaohsiung area in southern Taiwan .
	manualset3
156546	3	410132	7	NULL	NULL	0	NULL	abused women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey interview was used to collect data on abused women recruited from the Kaohsiung area in southern Taiwan .
	manualset3
156547	4	410132	7	NULL	NULL	0	NULL	Kaohsiung area in southern Taiwan	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey interview was used to collect data on abused women recruited from the Kaohsiung area in southern Taiwan .
	manualset3
156548	1	410133	7	NULL	NULL	0	NULL	following lectures	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The following lectures will be reviewed here : Jo-Ann Moulds -- Transfusion policies and practices in alloimmunized sickle cell patients ; Derwood Pamphilon -- Transfusion problems in stem cell transplant patients ; and Naomi Luban -- Transfusion issues in neonatal and pediatric hematology .
	manualset3
156549	2	410133	7	NULL	NULL	0	NULL	Jo-Ann Moulds -- Transfusion policies and practices in alloimmunized sickle cell patients	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The following lectures will be reviewed here : Jo-Ann Moulds -- Transfusion policies and practices in alloimmunized sickle cell patients ; Derwood Pamphilon -- Transfusion problems in stem cell transplant patients ; and Naomi Luban -- Transfusion issues in neonatal and pediatric hematology .
	manualset3
156550	3	410133	7	NULL	NULL	0	NULL	Derwood Pamphilon -- Transfusion problems in stem cell transplant patients	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The following lectures will be reviewed here : Jo-Ann Moulds -- Transfusion policies and practices in alloimmunized sickle cell patients ; Derwood Pamphilon -- Transfusion problems in stem cell transplant patients ; and Naomi Luban -- Transfusion issues in neonatal and pediatric hematology .
	manualset3
156551	4	410133	7	NULL	NULL	0	NULL	Naomi Luban -- Transfusion issues in neonatal and pediatric hematology	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The following lectures will be reviewed here : Jo-Ann Moulds -- Transfusion policies and practices in alloimmunized sickle cell patients ; Derwood Pamphilon -- Transfusion problems in stem cell transplant patients ; and Naomi Luban -- Transfusion issues in neonatal and pediatric hematology .
	manualset3
156552	1	410134	7	NULL	NULL	NULL	NULL	 magnetic parameters	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The following magnetic parameters were determined experimentally for ZnP / ( 67 ) ZnP , g ( ) = 1.9982 ( 2 ) , A ( ) ( P ) = 111 ( 6 ) MHz , A ( ) ( ( 67 ) Zn ) = 160 ( 2 ) MHz , and D = -29988 ( 3 ) MHz and estimates were made for the following ZnP / ( 67 ) ZnP magnetic parameters : g ( ) = 1.9941 ( 2 ) , A ( ) ( P ) = -5 ( 6 ) MHz , and A ( ) ( ( 67 ) Zn ) = 180 ( 50 ) MHz .
	manualset3
156554	2	410134	7	NULL	NULL	NULL	NULL	ZnP / ( 67 ) ZnP , g ( ) = 1.9982 ( 2 ) 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The following magnetic parameters were determined experimentally for ZnP / ( 67 ) ZnP , g ( ) = 1.9982 ( 2 ) , A ( ) ( P ) = 111 ( 6 ) MHz , A ( ) ( ( 67 ) Zn ) = 160 ( 2 ) MHz , and D = -29988 ( 3 ) MHz and estimates were made for the following ZnP / ( 67 ) ZnP magnetic parameters : g ( ) = 1.9941 ( 2 ) , A ( ) ( P ) = -5 ( 6 ) MHz , and A ( ) ( ( 67 ) Zn ) = 180 ( 50 ) MHz .
	manualset3
156555	3	410134	7	NULL	NULL	0	NULL	A ( ) ( P ) = 111 ( 6 ) MHz 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The following magnetic parameters were determined experimentally for ZnP / ( 67 ) ZnP , g ( ) = 1.9982 ( 2 ) , A ( ) ( P ) = 111 ( 6 ) MHz , A ( ) ( ( 67 ) Zn ) = 160 ( 2 ) MHz , and D = -29988 ( 3 ) MHz and estimates were made for the following ZnP / ( 67 ) ZnP magnetic parameters : g ( ) = 1.9941 ( 2 ) , A ( ) ( P ) = -5 ( 6 ) MHz , and A ( ) ( ( 67 ) Zn ) = 180 ( 50 ) MHz .
	manualset3
156556	4	410134	7	NULL	NULL	0	NULL	A ( ) ( ( 67 ) Zn ) = 160 ( 2 ) MHz	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The following magnetic parameters were determined experimentally for ZnP / ( 67 ) ZnP , g ( ) = 1.9982 ( 2 ) , A ( ) ( P ) = 111 ( 6 ) MHz , A ( ) ( ( 67 ) Zn ) = 160 ( 2 ) MHz , and D = -29988 ( 3 ) MHz and estimates were made for the following ZnP / ( 67 ) ZnP magnetic parameters : g ( ) = 1.9941 ( 2 ) , A ( ) ( P ) = -5 ( 6 ) MHz , and A ( ) ( ( 67 ) Zn ) = 180 ( 50 ) MHz .
	manualset3
156557	5	410134	7	NULL	NULL	0	NULL	D = -29988 ( 3 ) MHz 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The following magnetic parameters were determined experimentally for ZnP / ( 67 ) ZnP , g ( ) = 1.9982 ( 2 ) , A ( ) ( P ) = 111 ( 6 ) MHz , A ( ) ( ( 67 ) Zn ) = 160 ( 2 ) MHz , and D = -29988 ( 3 ) MHz and estimates were made for the following ZnP / ( 67 ) ZnP magnetic parameters : g ( ) = 1.9941 ( 2 ) , A ( ) ( P ) = -5 ( 6 ) MHz , and A ( ) ( ( 67 ) Zn ) = 180 ( 50 ) MHz .
	manualset3
156558	6	410134	7	NULL	NULL	0	NULL	ZnP / ( 67 ) ZnP magnetic parameters : g ( ) = 1.9941 ( 2 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The following magnetic parameters were determined experimentally for ZnP / ( 67 ) ZnP , g ( ) = 1.9982 ( 2 ) , A ( ) ( P ) = 111 ( 6 ) MHz , A ( ) ( ( 67 ) Zn ) = 160 ( 2 ) MHz , and D = -29988 ( 3 ) MHz and estimates were made for the following ZnP / ( 67 ) ZnP magnetic parameters : g ( ) = 1.9941 ( 2 ) , A ( ) ( P ) = -5 ( 6 ) MHz , and A ( ) ( ( 67 ) Zn ) = 180 ( 50 ) MHz .
	manualset3
156559	7	410134	7	NULL	NULL	0	NULL	A ( ) ( P ) = -5 ( 6 ) MHz	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The following magnetic parameters were determined experimentally for ZnP / ( 67 ) ZnP , g ( ) = 1.9982 ( 2 ) , A ( ) ( P ) = 111 ( 6 ) MHz , A ( ) ( ( 67 ) Zn ) = 160 ( 2 ) MHz , and D = -29988 ( 3 ) MHz and estimates were made for the following ZnP / ( 67 ) ZnP magnetic parameters : g ( ) = 1.9941 ( 2 ) , A ( ) ( P ) = -5 ( 6 ) MHz , and A ( ) ( ( 67 ) Zn ) = 180 ( 50 ) MHz .
	manualset3
156560	8	410134	7	NULL	NULL	0	NULL	A ( ) ( ( 67 ) Zn ) = 180 ( 50 ) MHz	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The following magnetic parameters were determined experimentally for ZnP / ( 67 ) ZnP , g ( ) = 1.9982 ( 2 ) , A ( ) ( P ) = 111 ( 6 ) MHz , A ( ) ( ( 67 ) Zn ) = 160 ( 2 ) MHz , and D = -29988 ( 3 ) MHz and estimates were made for the following ZnP / ( 67 ) ZnP magnetic parameters : g ( ) = 1.9941 ( 2 ) , A ( ) ( P ) = -5 ( 6 ) MHz , and A ( ) ( ( 67 ) Zn ) = 180 ( 50 ) MHz .
	manualset3
156561	1	410135	7	NULL	NULL	0	NULL	dramatic reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The following points can be made : ( 1 ) There is a dramatic reduction in the overall labeling of the crypt which begins within 3 h and is at its minimum by 15 h postirradiation .
	manualset3
156563	2	410135	7	NULL	NULL	0	NULL	overall labeling of the crypt 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The following points can be made : ( 1 ) There is a dramatic reduction in the overall labeling of the crypt which begins within 3 h and is at its minimum by 15 h postirradiation .
	manualset3
156564	3	410135	7	NULL	NULL	0	NULL	3 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The following points can be made : ( 1 ) There is a dramatic reduction in the overall labeling of the crypt which begins within 3 h and is at its minimum by 15 h postirradiation .
	manualset3
156565	5	410135	7	NULL	NULL	NULL	NULL	15 h postirradiation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The following points can be made : ( 1 ) There is a dramatic reduction in the overall labeling of the crypt which begins within 3 h and is at its minimum by 15 h postirradiation .
	manualset3
156566	4	410135	7	NULL	NULL	NULL	NULL	minimum	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The following points can be made : ( 1 ) There is a dramatic reduction in the overall labeling of the crypt which begins within 3 h and is at its minimum by 15 h postirradiation .
	manualset3
156567	1	410136	7	NULL	NULL	0	NULL	following recommendations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The following recommendations for therapy of parturients suffering from HELLP syndrome are given : epidural anesthesia is not an appropriate method in HELLP syndrome because of the risk of epidural hemorrhage due to thrombopenia .
	manualset3
156568	2	410136	7	NULL	NULL	0	NULL	therapy of parturients	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The following recommendations for therapy of parturients suffering from HELLP syndrome are given : epidural anesthesia is not an appropriate method in HELLP syndrome because of the risk of epidural hemorrhage due to thrombopenia .
	manualset3
156569	3	410136	7	NULL	NULL	0	NULL	HELLP syndrome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The following recommendations for therapy of parturients suffering from HELLP syndrome are given : epidural anesthesia is not an appropriate method in HELLP syndrome because of the risk of epidural hemorrhage due to thrombopenia .
	manualset3
156570	4	410136	7	NULL	NULL	NULL	NULL	epidural anesthesia 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The following recommendations for therapy of parturients suffering from HELLP syndrome are given : epidural anesthesia is not an appropriate method in HELLP syndrome because of the risk of epidural hemorrhage due to thrombopenia .
	manualset3
156571	5	410136	7	NULL	NULL	0	NULL	appropriate method	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The following recommendations for therapy of parturients suffering from HELLP syndrome are given : epidural anesthesia is not an appropriate method in HELLP syndrome because of the risk of epidural hemorrhage due to thrombopenia .
	manualset3
156572	6	410136	7	NULL	NULL	0	NULL	risk of epidural hemorrhage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The following recommendations for therapy of parturients suffering from HELLP syndrome are given : epidural anesthesia is not an appropriate method in HELLP syndrome because of the risk of epidural hemorrhage due to thrombopenia .
	manualset3
156573	7	410136	7	NULL	NULL	0	NULL	thrombopenia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The following recommendations for therapy of parturients suffering from HELLP syndrome are given : epidural anesthesia is not an appropriate method in HELLP syndrome because of the risk of epidural hemorrhage due to thrombopenia .
	manualset3
157311	8	410136	7	NULL	NULL	0	NULL	HELLP syndrome 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The following recommendations for therapy of parturients suffering from HELLP syndrome are given : epidural anesthesia is not an appropriate method in HELLP syndrome because of the risk of epidural hemorrhage due to thrombopenia .
	manualset3
156574	1	410137	7	NULL	NULL	0	NULL	following variables	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The following variables were studied , keeping the pressure controlled about 1200 p.s.i. : the extraction temperature , the time of static and dynamic extraction and the flow-rate of water ( 1 p.s.i. = 6894.76 Pa ) .
	manualset3
156575	2	410137	7	NULL	NULL	0	NULL	1200 p.s.i.	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The following variables were studied , keeping the pressure controlled about 1200 p.s.i. : the extraction temperature , the time of static and dynamic extraction and the flow-rate of water ( 1 p.s.i. = 6894.76 Pa ) .
	manualset3
156576	3	410137	7	NULL	NULL	0	NULL	extraction temperature	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The following variables were studied , keeping the pressure controlled about 1200 p.s.i. : the extraction temperature , the time of static and dynamic extraction and the flow-rate of water ( 1 p.s.i. = 6894.76 Pa ) .
	manualset3
156577	4	410137	7	NULL	NULL	0	NULL	time of static extraction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The following variables were studied , keeping the pressure controlled about 1200 p.s.i. : the extraction temperature , the time of static and dynamic extraction and the flow-rate of water ( 1 p.s.i. = 6894.76 Pa ) .
	manualset3
156578	5	410137	7	NULL	NULL	0	NULL	time of dynamic extraction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The following variables were studied , keeping the pressure controlled about 1200 p.s.i. : the extraction temperature , the time of static and dynamic extraction and the flow-rate of water ( 1 p.s.i. = 6894.76 Pa ) .
	manualset3
156579	6	410137	7	NULL	NULL	0	NULL	flow-rate of water	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The following variables were studied , keeping the pressure controlled about 1200 p.s.i. : the extraction temperature , the time of static and dynamic extraction and the flow-rate of water ( 1 p.s.i. = 6894.76 Pa ) .
	manualset3
156580	7	410137	7	NULL	NULL	0	NULL	1 p.s.i. = 6894.76 Pa 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The following variables were studied , keeping the pressure controlled about 1200 p.s.i. : the extraction temperature , the time of static and dynamic extraction and the flow-rate of water ( 1 p.s.i. = 6894.76 Pa ) .
	manualset3
157312	8	410137	7	NULL	NULL	0	NULL	pressure	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The following variables were studied , keeping the pressure controlled about 1200 p.s.i. : the extraction temperature , the time of static and dynamic extraction and the flow-rate of water ( 1 p.s.i. = 6894.76 Pa ) .
	manualset3
156581	1	410138	7	NULL	NULL	0	NULL	foods	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The foods to be analyzed were apricots , carrots , chickpeas , onions , raisins , and the sugar beet fiber Fibrex .
	manualset3
156582	2	410138	7	NULL	NULL	0	NULL	apricots	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The foods to be analyzed were apricots , carrots , chickpeas , onions , raisins , and the sugar beet fiber Fibrex .
	manualset3
156583	3	410138	7	NULL	NULL	0	NULL	carrots	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The foods to be analyzed were apricots , carrots , chickpeas , onions , raisins , and the sugar beet fiber Fibrex .
	manualset3
156584	4	410138	7	NULL	NULL	0	NULL	chickpeas	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The foods to be analyzed were apricots , carrots , chickpeas , onions , raisins , and the sugar beet fiber Fibrex .
	manualset3
156585	5	410138	7	NULL	NULL	0	NULL	onions	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The foods to be analyzed were apricots , carrots , chickpeas , onions , raisins , and the sugar beet fiber Fibrex .
	manualset3
156586	6	410138	7	NULL	NULL	0	NULL	 raisins 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The foods to be analyzed were apricots , carrots , chickpeas , onions , raisins , and the sugar beet fiber Fibrex .
	manualset3
156587	7	410138	7	NULL	NULL	0	NULL	sugar beet fiber Fibrex	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The foods to be analyzed were apricots , carrots , chickpeas , onions , raisins , and the sugar beet fiber Fibrex .
	manualset3
156588	1	410139	7	NULL	NULL	0	NULL	force-frequency relation 	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The force-frequency relation was significantly depressed at 120 min of reperfusion in both groups , but optimal heart rate was significantly lower in the control group ( P = 0.04 ) .
	manualset3
156589	2	410139	7	NULL	NULL	0	NULL	120 min of reperfusion	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The force-frequency relation was significantly depressed at 120 min of reperfusion in both groups , but optimal heart rate was significantly lower in the control group ( P = 0.04 ) .
	manualset3
156590	3	410139	7	NULL	NULL	0	NULL	groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The force-frequency relation was significantly depressed at 120 min of reperfusion in both groups , but optimal heart rate was significantly lower in the control group ( P = 0.04 ) .
	manualset3
156591	4	410139	7	NULL	NULL	NULL	NULL	optimal heart rate	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The force-frequency relation was significantly depressed at 120 min of reperfusion in both groups , but optimal heart rate was significantly lower in the control group ( P = 0.04 ) .
	manualset3
156592	5	410139	7	NULL	NULL	0	NULL	control group 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The force-frequency relation was significantly depressed at 120 min of reperfusion in both groups , but optimal heart rate was significantly lower in the control group ( P = 0.04 ) .
	manualset3
156593	6	410139	7	NULL	NULL	0	NULL	P = 0.04	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The force-frequency relation was significantly depressed at 120 min of reperfusion in both groups , but optimal heart rate was significantly lower in the control group ( P = 0.04 ) .
	manualset3
157313	7	410139	7	NULL	NULL	0	NULL	force-frequency relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The force-frequency relation was significantly depressed at 120 min of reperfusion in both groups , but optimal heart rate was significantly lower in the control group ( P = 0.04 ) .
	manualset3
156594	1	410140	7	NULL	NULL	0	NULL	 force and displacement	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The force and displacement at yield , stiffness and ultimate force were determined for 4 repair techniques based on an acrylic material , polyurethane patch attached with cyanoacrylate adhesive , steel plate attached with screws and a transverse metal bar cut into the hoof wall .
	manualset3
156595	3	410140	7	NULL	NULL	NULL	NULL	stiffness 	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The force and displacement at yield , stiffness and ultimate force were determined for 4 repair techniques based on an acrylic material , polyurethane patch attached with cyanoacrylate adhesive , steel plate attached with screws and a transverse metal bar cut into the hoof wall .
	manualset3
156596	2	410140	7	NULL	NULL	NULL	NULL	yield	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The force and displacement at yield , stiffness and ultimate force were determined for 4 repair techniques based on an acrylic material , polyurethane patch attached with cyanoacrylate adhesive , steel plate attached with screws and a transverse metal bar cut into the hoof wall .
	manualset3
156598	5	410140	7	NULL	NULL	0	NULL	4 repair techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The force and displacement at yield , stiffness and ultimate force were determined for 4 repair techniques based on an acrylic material , polyurethane patch attached with cyanoacrylate adhesive , steel plate attached with screws and a transverse metal bar cut into the hoof wall .
	manualset3
156599	6	410140	7	NULL	NULL	0	NULL	acrylic material	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The force and displacement at yield , stiffness and ultimate force were determined for 4 repair techniques based on an acrylic material , polyurethane patch attached with cyanoacrylate adhesive , steel plate attached with screws and a transverse metal bar cut into the hoof wall .
	manualset3
156600	7	410140	7	NULL	NULL	NULL	NULL	polyurethane patch attached with cyanoacrylate adhesive	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The force and displacement at yield , stiffness and ultimate force were determined for 4 repair techniques based on an acrylic material , polyurethane patch attached with cyanoacrylate adhesive , steel plate attached with screws and a transverse metal bar cut into the hoof wall .
	manualset3
156602	9	410140	7	NULL	NULL	0	NULL	steel plate attached with screws 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The force and displacement at yield , stiffness and ultimate force were determined for 4 repair techniques based on an acrylic material , polyurethane patch attached with cyanoacrylate adhesive , steel plate attached with screws and a transverse metal bar cut into the hoof wall .
	manualset3
156603	10	410140	7	NULL	NULL	0	NULL	transverse metal bar cut into the hoof wall	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The force and displacement at yield , stiffness and ultimate force were determined for 4 repair techniques based on an acrylic material , polyurethane patch attached with cyanoacrylate adhesive , steel plate attached with screws and a transverse metal bar cut into the hoof wall .
	manualset3
157314	11	410140	7	NULL	NULL	0	NULL	ultimate force	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The force and displacement at yield , stiffness and ultimate force were determined for 4 repair techniques based on an acrylic material , polyurethane patch attached with cyanoacrylate adhesive , steel plate attached with screws and a transverse metal bar cut into the hoof wall .
	manualset3
156604	1	410141	7	NULL	NULL	0	NULL	force	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The force imposed on the cells was measured directly during compression to various deformations and then holding .
	manualset3
156605	2	410141	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The force imposed on the cells was measured directly during compression to various deformations and then holding .
	manualset3
156606	3	410141	7	NULL	NULL	0	NULL	compression	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The force imposed on the cells was measured directly during compression to various deformations and then holding .
	manualset3
156607	4	410141	7	NULL	NULL	0	NULL	deformations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The force imposed on the cells was measured directly during compression to various deformations and then holding .
	manualset3
156608	1	410142	7	NULL	NULL	0	NULL	survey	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey of 15 publicly-funded treatment agencies in Iowa was conducted to identify correlates of satisfaction with substance abuse treatment for voluntary clients .
	manualset3
156609	2	410142	7	NULL	NULL	0	NULL	15 publicly-funded treatment agencies	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey of 15 publicly-funded treatment agencies in Iowa was conducted to identify correlates of satisfaction with substance abuse treatment for voluntary clients .
	manualset3
156610	3	410142	7	NULL	NULL	0	NULL	 Iowa	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey of 15 publicly-funded treatment agencies in Iowa was conducted to identify correlates of satisfaction with substance abuse treatment for voluntary clients .
	manualset3
156612	4	410142	7	NULL	NULL	NULL	NULL	substance abuse treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A survey of 15 publicly-funded treatment agencies in Iowa was conducted to identify correlates of satisfaction with substance abuse treatment for voluntary clients .
	manualset3
156613	5	410142	7	NULL	NULL	0	NULL	voluntary clients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey of 15 publicly-funded treatment agencies in Iowa was conducted to identify correlates of satisfaction with substance abuse treatment for voluntary clients .
	manualset3
157315	6	410142	7	NULL	NULL	0	NULL	satisfaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey of 15 publicly-funded treatment agencies in Iowa was conducted to identify correlates of satisfaction with substance abuse treatment for voluntary clients .
	manualset3
157316	7	410142	7	NULL	NULL	0	NULL	correlates	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey of 15 publicly-funded treatment agencies in Iowa was conducted to identify correlates of satisfaction with substance abuse treatment for voluntary clients .
	manualset3
156614	1	410143	7	NULL	NULL	NULL	NULL	formal potential of Mb	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The formal potential of Mb on Cys SAM exhibited pH-dependent variation in the pH range of 5-9 with a slope of 55 mV/pH , indicating that the electron transfer is accompanied by a single proton exchange .
	manualset3
156615	2	410143	7	NULL	NULL	0	NULL	Cys SAM	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The formal potential of Mb on Cys SAM exhibited pH-dependent variation in the pH range of 5-9 with a slope of 55 mV/pH , indicating that the electron transfer is accompanied by a single proton exchange .
	manualset3
156616	3	410143	7	NULL	NULL	0	NULL	pH-dependent variation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The formal potential of Mb on Cys SAM exhibited pH-dependent variation in the pH range of 5-9 with a slope of 55 mV/pH , indicating that the electron transfer is accompanied by a single proton exchange .
	manualset3
156617	4	410143	7	NULL	NULL	0	NULL	pH range of 5-9	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The formal potential of Mb on Cys SAM exhibited pH-dependent variation in the pH range of 5-9 with a slope of 55 mV/pH , indicating that the electron transfer is accompanied by a single proton exchange .
	manualset3
156618	5	410143	7	NULL	NULL	0	NULL	slope of 55 mV/pH	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The formal potential of Mb on Cys SAM exhibited pH-dependent variation in the pH range of 5-9 with a slope of 55 mV/pH , indicating that the electron transfer is accompanied by a single proton exchange .
	manualset3
156619	6	410143	7	NULL	NULL	0	NULL	electron transfer 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The formal potential of Mb on Cys SAM exhibited pH-dependent variation in the pH range of 5-9 with a slope of 55 mV/pH , indicating that the electron transfer is accompanied by a single proton exchange .
	manualset3
156620	7	410143	7	NULL	NULL	0	NULL	single proton exchange	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The formal potential of Mb on Cys SAM exhibited pH-dependent variation in the pH range of 5-9 with a slope of 55 mV/pH , indicating that the electron transfer is accompanied by a single proton exchange .
	manualset3
156621	1	410144	7	NULL	NULL	NULL	NULL	formation constant	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The formation constant dramatically increases with the length of n-alkyl , it starts from the value of 140 l mol ( -1 ) for the phenanthrene to reach the value of 580 l mol ( -1 ) for hexyl-phenanthrene .
	manualset3
156622	2	410144	7	NULL	NULL	0	NULL	 length of n-alkyl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation constant dramatically increases with the length of n-alkyl , it starts from the value of 140 l mol ( -1 ) for the phenanthrene to reach the value of 580 l mol ( -1 ) for hexyl-phenanthrene .
	manualset3
156623	3	410144	7	NULL	NULL	NULL	NULL	140 l mol ( -1 ) 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The formation constant dramatically increases with the length of n-alkyl , it starts from the value of 140 l mol ( -1 ) for the phenanthrene to reach the value of 580 l mol ( -1 ) for hexyl-phenanthrene .
	manualset3
156624	4	410144	7	NULL	NULL	0	NULL	phenanthrene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation constant dramatically increases with the length of n-alkyl , it starts from the value of 140 l mol ( -1 ) for the phenanthrene to reach the value of 580 l mol ( -1 ) for hexyl-phenanthrene .
	manualset3
156625	5	410144	7	NULL	NULL	0	NULL	580 l mol ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation constant dramatically increases with the length of n-alkyl , it starts from the value of 140 l mol ( -1 ) for the phenanthrene to reach the value of 580 l mol ( -1 ) for hexyl-phenanthrene .
	manualset3
156626	6	410144	7	NULL	NULL	0	NULL	hexyl-phenanthrene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation constant dramatically increases with the length of n-alkyl , it starts from the value of 140 l mol ( -1 ) for the phenanthrene to reach the value of 580 l mol ( -1 ) for hexyl-phenanthrene .
	manualset3
157317	7	410144	7	NULL	NULL	0	NULL	value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation constant dramatically increases with the length of n-alkyl , it starts from the value of 140 l mol ( -1 ) for the phenanthrene to reach the value of 580 l mol ( -1 ) for hexyl-phenanthrene .
	manualset3
156627	1	410145	7	NULL	NULL	0	NULL	formation of 150-kDa complexes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation of 150-kDa complexes containing hIGFBP-3 was not accompanied by a corresponding change in the IGF-I content ( determined by RIA ) of whole serum or 150-kDa serum fractions , suggesting that the hIGFBP-3 had rapidly associated with rALS in vivo without mobilizing IGF-I .
	manualset3
156628	2	410145	7	NULL	NULL	0	NULL	hIGFBP-3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation of 150-kDa complexes containing hIGFBP-3 was not accompanied by a corresponding change in the IGF-I content ( determined by RIA ) of whole serum or 150-kDa serum fractions , suggesting that the hIGFBP-3 had rapidly associated with rALS in vivo without mobilizing IGF-I .
	manualset3
156629	3	410145	7	NULL	NULL	0	NULL	IGF-I content	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation of 150-kDa complexes containing hIGFBP-3 was not accompanied by a corresponding change in the IGF-I content ( determined by RIA ) of whole serum or 150-kDa serum fractions , suggesting that the hIGFBP-3 had rapidly associated with rALS in vivo without mobilizing IGF-I .
	manualset3
156630	4	410145	7	NULL	NULL	0	NULL	RIA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation of 150-kDa complexes containing hIGFBP-3 was not accompanied by a corresponding change in the IGF-I content ( determined by RIA ) of whole serum or 150-kDa serum fractions , suggesting that the hIGFBP-3 had rapidly associated with rALS in vivo without mobilizing IGF-I .
	manualset3
156631	5	410145	7	NULL	NULL	0	NULL	whole serum 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation of 150-kDa complexes containing hIGFBP-3 was not accompanied by a corresponding change in the IGF-I content ( determined by RIA ) of whole serum or 150-kDa serum fractions , suggesting that the hIGFBP-3 had rapidly associated with rALS in vivo without mobilizing IGF-I .
	manualset3
156632	6	410145	7	NULL	NULL	0	NULL	150-kDa serum fractions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation of 150-kDa complexes containing hIGFBP-3 was not accompanied by a corresponding change in the IGF-I content ( determined by RIA ) of whole serum or 150-kDa serum fractions , suggesting that the hIGFBP-3 had rapidly associated with rALS in vivo without mobilizing IGF-I .
	manualset3
156633	7	410145	7	NULL	NULL	0	NULL	hIGFBP-3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation of 150-kDa complexes containing hIGFBP-3 was not accompanied by a corresponding change in the IGF-I content ( determined by RIA ) of whole serum or 150-kDa serum fractions , suggesting that the hIGFBP-3 had rapidly associated with rALS in vivo without mobilizing IGF-I .
	manualset3
156634	8	410145	7	NULL	NULL	0	NULL	rALS	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation of 150-kDa complexes containing hIGFBP-3 was not accompanied by a corresponding change in the IGF-I content ( determined by RIA ) of whole serum or 150-kDa serum fractions , suggesting that the hIGFBP-3 had rapidly associated with rALS in vivo without mobilizing IGF-I .
	manualset3
156635	9	410145	7	NULL	NULL	0	NULL	in vivo	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation of 150-kDa complexes containing hIGFBP-3 was not accompanied by a corresponding change in the IGF-I content ( determined by RIA ) of whole serum or 150-kDa serum fractions , suggesting that the hIGFBP-3 had rapidly associated with rALS in vivo without mobilizing IGF-I .
	manualset3
156636	10	410145	7	NULL	NULL	0	NULL	IGF-I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation of 150-kDa complexes containing hIGFBP-3 was not accompanied by a corresponding change in the IGF-I content ( determined by RIA ) of whole serum or 150-kDa serum fractions , suggesting that the hIGFBP-3 had rapidly associated with rALS in vivo without mobilizing IGF-I .
	manualset3
156637	1	410146	7	NULL	NULL	0	NULL	formation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation of a deletion derivative of plasmid pBR322 , designated pBR322 delta 1 , was observed during cloning of various eukaryotic DNAs , when the BamHI site of the plasmid vector was used for construction of the recombinant molecules .
	manualset3
156638	2	410146	7	NULL	NULL	NULL	NULL	deletion derivative of plasmid pBR322	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The formation of a deletion derivative of plasmid pBR322 , designated pBR322 delta 1 , was observed during cloning of various eukaryotic DNAs , when the BamHI site of the plasmid vector was used for construction of the recombinant molecules .
	manualset3
156639	3	410146	7	NULL	NULL	0	NULL	pBR322 delta 1	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation of a deletion derivative of plasmid pBR322 , designated pBR322 delta 1 , was observed during cloning of various eukaryotic DNAs , when the BamHI site of the plasmid vector was used for construction of the recombinant molecules .
	manualset3
156640	4	410146	7	NULL	NULL	NULL	NULL	 eukaryotic DNAs	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The formation of a deletion derivative of plasmid pBR322 , designated pBR322 delta 1 , was observed during cloning of various eukaryotic DNAs , when the BamHI site of the plasmid vector was used for construction of the recombinant molecules .
	manualset3
156641	5	410146	7	NULL	NULL	0	NULL	BamHI site of the plasmid vector 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation of a deletion derivative of plasmid pBR322 , designated pBR322 delta 1 , was observed during cloning of various eukaryotic DNAs , when the BamHI site of the plasmid vector was used for construction of the recombinant molecules .
	manualset3
156642	6	410146	7	NULL	NULL	0	NULL	recombinant molecules 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation of a deletion derivative of plasmid pBR322 , designated pBR322 delta 1 , was observed during cloning of various eukaryotic DNAs , when the BamHI site of the plasmid vector was used for construction of the recombinant molecules .
	manualset3
157318	7	410146	7	NULL	NULL	0	NULL	cloning	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation of a deletion derivative of plasmid pBR322 , designated pBR322 delta 1 , was observed during cloning of various eukaryotic DNAs , when the BamHI site of the plasmid vector was used for construction of the recombinant molecules .
	manualset3
157319	8	410146	7	NULL	NULL	0	NULL	construction	R												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation of a deletion derivative of plasmid pBR322 , designated pBR322 delta 1 , was observed during cloning of various eukaryotic DNAs , when the BamHI site of the plasmid vector was used for construction of the recombinant molecules .
	manualset3
156643	1	410147	7	NULL	NULL	NULL	NULL	former	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The former focuses on mental stabilization , strengthening of the ego , and improved adjustment to the trauma and its effects .
	manualset3
156644	2	410147	7	NULL	NULL	NULL	NULL	mental stabilization 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The former focuses on mental stabilization , strengthening of the ego , and improved adjustment to the trauma and its effects .
	manualset3
156645	3	410147	7	NULL	NULL	0	NULL	strengthening of the ego	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The former focuses on mental stabilization , strengthening of the ego , and improved adjustment to the trauma and its effects .
	manualset3
156646	4	410147	7	NULL	NULL	0	NULL	 trauma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The former focuses on mental stabilization , strengthening of the ego , and improved adjustment to the trauma and its effects .
	manualset3
156647	5	410147	7	NULL	NULL	0	NULL	effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The former focuses on mental stabilization , strengthening of the ego , and improved adjustment to the trauma and its effects .
	manualset3
157320	6	410147	7	NULL	NULL	0	NULL	adjustment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The former focuses on mental stabilization , strengthening of the ego , and improved adjustment to the trauma and its effects .
	manualset3
156648	1	410148	7	NULL	NULL	NULL	NULL	former 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The former is able to extract knowledge from data using a symbolic-numeric machine learning system , and the latter is able to control the learning process by accepting and validating the machine results , or by criticizing those results or the explanation that the system produces on them .
	manualset3
156649	2	410148	7	NULL	NULL	0	NULL	extract knowledge from data	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The former is able to extract knowledge from data using a symbolic-numeric machine learning system , and the latter is able to control the learning process by accepting and validating the machine results , or by criticizing those results or the explanation that the system produces on them .
	manualset3
156650	3	410148	7	NULL	NULL	0	NULL	symbolic-numeric machine learning system	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The former is able to extract knowledge from data using a symbolic-numeric machine learning system , and the latter is able to control the learning process by accepting and validating the machine results , or by criticizing those results or the explanation that the system produces on them .
	manualset3
156651	4	410148	7	NULL	NULL	NULL	NULL	learning process	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The former is able to extract knowledge from data using a symbolic-numeric machine learning system , and the latter is able to control the learning process by accepting and validating the machine results , or by criticizing those results or the explanation that the system produces on them .
	manualset3
156652	5	410148	7	NULL	NULL	0	NULL	machine results	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The former is able to extract knowledge from data using a symbolic-numeric machine learning system , and the latter is able to control the learning process by accepting and validating the machine results , or by criticizing those results or the explanation that the system produces on them .
	manualset3
156653	6	410148	7	NULL	NULL	0	NULL	 system	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The former is able to extract knowledge from data using a symbolic-numeric machine learning system , and the latter is able to control the learning process by accepting and validating the machine results , or by criticizing those results or the explanation that the system produces on them .
	manualset3
157321	7	410148	7	NULL	NULL	0	NULL	results	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The former is able to extract knowledge from data using a symbolic-numeric machine learning system , and the latter is able to control the learning process by accepting and validating the machine results , or by criticizing those results or the explanation that the system produces on them .
	manualset3
157322	8	410148	7	NULL	NULL	0	NULL	explanation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The former is able to extract knowledge from data using a symbolic-numeric machine learning system , and the latter is able to control the learning process by accepting and validating the machine results , or by criticizing those results or the explanation that the system produces on them .
	manualset3
156654	1	410149	7	NULL	NULL	NULL	NULL	former method	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The former method , based on the Von Kries color conversion in the CIE xyY color space , retrieves the original color of the paint paper by modifying colors based on their similarity to the background color .
	manualset3
156655	2	410149	7	NULL	NULL	0	NULL	Von Kries color conversion	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The former method , based on the Von Kries color conversion in the CIE xyY color space , retrieves the original color of the paint paper by modifying colors based on their similarity to the background color .
	manualset3
156656	3	410149	7	NULL	NULL	0	NULL	CIE xyY color space	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The former method , based on the Von Kries color conversion in the CIE xyY color space , retrieves the original color of the paint paper by modifying colors based on their similarity to the background color .
	manualset3
156657	4	410149	7	NULL	NULL	NULL	NULL	original color of the paint paper	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The former method , based on the Von Kries color conversion in the CIE xyY color space , retrieves the original color of the paint paper by modifying colors based on their similarity to the background color .
	manualset3
156658	5	410149	7	NULL	NULL	0	NULL	colors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The former method , based on the Von Kries color conversion in the CIE xyY color space , retrieves the original color of the paint paper by modifying colors based on their similarity to the background color .
	manualset3
156659	6	410149	7	NULL	NULL	0	NULL	background color	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The former method , based on the Von Kries color conversion in the CIE xyY color space , retrieves the original color of the paint paper by modifying colors based on their similarity to the background color .
	manualset3
156660	1	410150	7	NULL	NULL	0	NULL	former technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The former technique described in detailed here offers substantial benefits in terms of measurement time and operator dependency , while not sacrificing the accuracy of the measurement .
	manualset3
156661	2	410150	7	NULL	NULL	0	NULL	substantial benefits	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The former technique described in detailed here offers substantial benefits in terms of measurement time and operator dependency , while not sacrificing the accuracy of the measurement .
	manualset3
156662	3	410150	7	NULL	NULL	0	NULL	measurement time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The former technique described in detailed here offers substantial benefits in terms of measurement time and operator dependency , while not sacrificing the accuracy of the measurement .
	manualset3
156663	4	410150	7	NULL	NULL	NULL	NULL	operator dependency	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The former technique described in detailed here offers substantial benefits in terms of measurement time and operator dependency , while not sacrificing the accuracy of the measurement .
	manualset3
156664	5	410150	7	NULL	NULL	0	NULL	accuracy of the measurement	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The former technique described in detailed here offers substantial benefits in terms of measurement time and operator dependency , while not sacrificing the accuracy of the measurement .
	manualset3
156665	1	410151	7	NULL	NULL	0	NULL	four elements	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The four elements found to be important to the creation of the Total Quality Management ( TQM ) environment were change in management culture , development of teamwork , focus on customers , and continuous feedback to staff .
	manualset3
156666	2	410151	7	NULL	NULL	NULL	NULL	creation of the Total Quality Management ( TQM ) environment	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The four elements found to be important to the creation of the Total Quality Management ( TQM ) environment were change in management culture , development of teamwork , focus on customers , and continuous feedback to staff .
	manualset3
156667	3	410151	7	NULL	NULL	0	NULL	management culture	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The four elements found to be important to the creation of the Total Quality Management ( TQM ) environment were change in management culture , development of teamwork , focus on customers , and continuous feedback to staff .
	manualset3
156668	4	410151	7	NULL	NULL	0	NULL	development of teamwork	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The four elements found to be important to the creation of the Total Quality Management ( TQM ) environment were change in management culture , development of teamwork , focus on customers , and continuous feedback to staff .
	manualset3
156669	5	410151	7	NULL	NULL	0	NULL	focus on customers	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The four elements found to be important to the creation of the Total Quality Management ( TQM ) environment were change in management culture , development of teamwork , focus on customers , and continuous feedback to staff .
	manualset3
156670	6	410151	7	NULL	NULL	0	NULL	continuous feedback to staff	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The four elements found to be important to the creation of the Total Quality Management ( TQM ) environment were change in management culture , development of teamwork , focus on customers , and continuous feedback to staff .
	manualset3
156671	1	410152	7	NULL	NULL	0	NULL	four leading malformations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The four leading malformations were pes-equinovarus 7 cases ( 9.1 % ) , labiognathopalatoschizis , hydrocephalus and anencephalus 6 cases each ( 7.7 % ) .
	manualset3
156672	2	410152	7	NULL	NULL	0	NULL	pes-equinovarus 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The four leading malformations were pes-equinovarus 7 cases ( 9.1 % ) , labiognathopalatoschizis , hydrocephalus and anencephalus 6 cases each ( 7.7 % ) .
	manualset3
156673	3	410152	7	NULL	NULL	0	NULL	 7 cases ( 9.1 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The four leading malformations were pes-equinovarus 7 cases ( 9.1 % ) , labiognathopalatoschizis , hydrocephalus and anencephalus 6 cases each ( 7.7 % ) .
	manualset3
156674	4	410152	7	NULL	NULL	0	NULL	 labiognathopalatoschizis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The four leading malformations were pes-equinovarus 7 cases ( 9.1 % ) , labiognathopalatoschizis , hydrocephalus and anencephalus 6 cases each ( 7.7 % ) .
	manualset3
156675	5	410152	7	NULL	NULL	0	NULL	hydrocephalus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The four leading malformations were pes-equinovarus 7 cases ( 9.1 % ) , labiognathopalatoschizis , hydrocephalus and anencephalus 6 cases each ( 7.7 % ) .
	manualset3
156676	6	410152	7	NULL	NULL	0	NULL	anencephalus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The four leading malformations were pes-equinovarus 7 cases ( 9.1 % ) , labiognathopalatoschizis , hydrocephalus and anencephalus 6 cases each ( 7.7 % ) .
	manualset3
156677	7	410152	7	NULL	NULL	0	NULL	6 cases  ( 7.7 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The four leading malformations were pes-equinovarus 7 cases ( 9.1 % ) , labiognathopalatoschizis , hydrocephalus and anencephalus 6 cases each ( 7.7 % ) .
	manualset3
156678	1	410153	7	NULL	NULL	0	NULL	four patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The four patients with pretreatment TTV DNA titer ) or = 10 ( 3 ) / ml did not respond .
	manualset3
156679	2	410153	7	NULL	NULL	NULL	NULL	pretreatment TTV DNA titer )	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The four patients with pretreatment TTV DNA titer ) or = 10 ( 3 ) / ml did not respond .
	manualset3
156680	3	410153	7	NULL	NULL	0	NULL	 10 ( 3 ) / ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The four patients with pretreatment TTV DNA titer ) or = 10 ( 3 ) / ml did not respond .
	manualset3
156681	1	410154	7	NULL	NULL	0	NULL	CSL4	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The fourth , CSL4 , corresponded to ORF YNL232w on chromosome XIV , and was found to be essential .
	manualset3
156682	2	410154	7	NULL	NULL	0	NULL	ORF YNL232w	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The fourth , CSL4 , corresponded to ORF YNL232w on chromosome XIV , and was found to be essential .
	manualset3
156683	3	410154	7	NULL	NULL	0	NULL	chromosome XIV 	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The fourth , CSL4 , corresponded to ORF YNL232w on chromosome XIV , and was found to be essential .
	manualset3
156684	1	410155	7	NULL	NULL	0	NULL	fourth patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The fourth patient had a lymphocytic lymphoma of B-cell origin in the inguinal lymph nodes which was treated with radiotherapy .
	manualset3
156685	2	410155	7	NULL	NULL	0	NULL	lymphocytic lymphoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The fourth patient had a lymphocytic lymphoma of B-cell origin in the inguinal lymph nodes which was treated with radiotherapy .
	manualset3
156686	3	410155	7	NULL	NULL	0	NULL	B-cell origin	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The fourth patient had a lymphocytic lymphoma of B-cell origin in the inguinal lymph nodes which was treated with radiotherapy .
	manualset3
156687	4	410155	7	NULL	NULL	0	NULL	inguinal lymph nodes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The fourth patient had a lymphocytic lymphoma of B-cell origin in the inguinal lymph nodes which was treated with radiotherapy .
	manualset3
156688	5	410155	7	NULL	NULL	NULL	NULL	radiotherapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fourth patient had a lymphocytic lymphoma of B-cell origin in the inguinal lymph nodes which was treated with radiotherapy .
	manualset3
156689	1	410156	7	NULL	NULL	0	NULL	survey	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey of benign hepatocellular tumors in a metropolitan area included six cases of hepatocellular adenoma , eight of focal nodular hyperplasia , and two of nodular transformation .
	manualset3
156690	2	410156	7	NULL	NULL	NULL	NULL	benign hepatocellular tumors	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A survey of benign hepatocellular tumors in a metropolitan area included six cases of hepatocellular adenoma , eight of focal nodular hyperplasia , and two of nodular transformation .
	manualset3
156691	3	410156	7	NULL	NULL	0	NULL	metropolitan area	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey of benign hepatocellular tumors in a metropolitan area included six cases of hepatocellular adenoma , eight of focal nodular hyperplasia , and two of nodular transformation .
	manualset3
156692	4	410156	7	NULL	NULL	0	NULL	six cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey of benign hepatocellular tumors in a metropolitan area included six cases of hepatocellular adenoma , eight of focal nodular hyperplasia , and two of nodular transformation .
	manualset3
156693	5	410156	7	NULL	NULL	NULL	NULL	hepatocellular adenoma	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A survey of benign hepatocellular tumors in a metropolitan area included six cases of hepatocellular adenoma , eight of focal nodular hyperplasia , and two of nodular transformation .
	manualset3
156694	6	410156	7	NULL	NULL	NULL	NULL	eight of focal nodular hyperplasia 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A survey of benign hepatocellular tumors in a metropolitan area included six cases of hepatocellular adenoma , eight of focal nodular hyperplasia , and two of nodular transformation .
	manualset3
156695	7	410156	7	NULL	NULL	0	NULL	two of nodular transformation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey of benign hepatocellular tumors in a metropolitan area included six cases of hepatocellular adenoma , eight of focal nodular hyperplasia , and two of nodular transformation .
	manualset3
156696	1	410157	7	NULL	NULL	0	NULL	fraction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The fraction with anticoagulant activity was purified from the spine venom of Acanthaster planci by fractionation with ammonium sulfate followed by column chromatography and designated plancinin .
	manualset3
156697	2	410157	7	NULL	NULL	0	NULL	anticoagulant activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The fraction with anticoagulant activity was purified from the spine venom of Acanthaster planci by fractionation with ammonium sulfate followed by column chromatography and designated plancinin .
	manualset3
156698	3	410157	7	NULL	NULL	0	NULL	spine venom	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The fraction with anticoagulant activity was purified from the spine venom of Acanthaster planci by fractionation with ammonium sulfate followed by column chromatography and designated plancinin .
	manualset3
156699	4	410157	7	NULL	NULL	0	NULL	Acanthaster planci	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The fraction with anticoagulant activity was purified from the spine venom of Acanthaster planci by fractionation with ammonium sulfate followed by column chromatography and designated plancinin .
	manualset3
156700	5	410157	7	NULL	NULL	0	NULL	ammonium sulfate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The fraction with anticoagulant activity was purified from the spine venom of Acanthaster planci by fractionation with ammonium sulfate followed by column chromatography and designated plancinin .
	manualset3
156701	6	410157	7	NULL	NULL	0	NULL	column chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The fraction with anticoagulant activity was purified from the spine venom of Acanthaster planci by fractionation with ammonium sulfate followed by column chromatography and designated plancinin .
	manualset3
156702	7	410157	7	NULL	NULL	0	NULL	plancinin	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The fraction with anticoagulant activity was purified from the spine venom of Acanthaster planci by fractionation with ammonium sulfate followed by column chromatography and designated plancinin .
	manualset3
157323	8	410157	7	NULL	NULL	0	NULL	fractionation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The fraction with anticoagulant activity was purified from the spine venom of Acanthaster planci by fractionation with ammonium sulfate followed by column chromatography and designated plancinin .
	manualset3
156703	1	410158	7	NULL	NULL	0	NULL	fractional rate	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The fractional rate of skeletal muscle protein synthesis and the whole body rate of protein breakdown were determined during a constant intravenous infusion of ( 13C ) leucine in 7 young ( 23 + / - 2 yr ; 86.2 + / - 4.6 kg ) healthy experienced male weight lifters before and at the end of 14 days of subcutaneous GH administration ( 40 microgram.kg-1 x day-1 ) .
	manualset3
156704	2	410158	7	NULL	NULL	0	NULL	skeletal muscle protein synthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The fractional rate of skeletal muscle protein synthesis and the whole body rate of protein breakdown were determined during a constant intravenous infusion of ( 13C ) leucine in 7 young ( 23 + / - 2 yr ; 86.2 + / - 4.6 kg ) healthy experienced male weight lifters before and at the end of 14 days of subcutaneous GH administration ( 40 microgram.kg-1 x day-1 ) .
	manualset3
156705	3	410158	7	NULL	NULL	0	NULL	whole body rate of protein breakdown	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The fractional rate of skeletal muscle protein synthesis and the whole body rate of protein breakdown were determined during a constant intravenous infusion of ( 13C ) leucine in 7 young ( 23 + / - 2 yr ; 86.2 + / - 4.6 kg ) healthy experienced male weight lifters before and at the end of 14 days of subcutaneous GH administration ( 40 microgram.kg-1 x day-1 ) .
	manualset3
156706	4	410158	7	NULL	NULL	0	NULL	constant intravenous infusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The fractional rate of skeletal muscle protein synthesis and the whole body rate of protein breakdown were determined during a constant intravenous infusion of ( 13C ) leucine in 7 young ( 23 + / - 2 yr ; 86.2 + / - 4.6 kg ) healthy experienced male weight lifters before and at the end of 14 days of subcutaneous GH administration ( 40 microgram.kg-1 x day-1 ) .
	manualset3
156707	5	410158	7	NULL	NULL	0	NULL	( 13C ) leucine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The fractional rate of skeletal muscle protein synthesis and the whole body rate of protein breakdown were determined during a constant intravenous infusion of ( 13C ) leucine in 7 young ( 23 + / - 2 yr ; 86.2 + / - 4.6 kg ) healthy experienced male weight lifters before and at the end of 14 days of subcutaneous GH administration ( 40 microgram.kg-1 x day-1 ) .
	manualset3
156708	6	410158	7	NULL	NULL	NULL	NULL	 7 young ( 23 + / - 2 yr ; 86.2 + / - 4.6 kg ) 	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fractional rate of skeletal muscle protein synthesis and the whole body rate of protein breakdown were determined during a constant intravenous infusion of ( 13C ) leucine in 7 young ( 23 + / - 2 yr ; 86.2 + / - 4.6 kg ) healthy experienced male weight lifters before and at the end of 14 days of subcutaneous GH administration ( 40 microgram.kg-1 x day-1 ) .
	manualset3
156709	7	410158	7	NULL	NULL	0	NULL	healthy experienced male weight lifters	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The fractional rate of skeletal muscle protein synthesis and the whole body rate of protein breakdown were determined during a constant intravenous infusion of ( 13C ) leucine in 7 young ( 23 + / - 2 yr ; 86.2 + / - 4.6 kg ) healthy experienced male weight lifters before and at the end of 14 days of subcutaneous GH administration ( 40 microgram.kg-1 x day-1 ) .
	manualset3
156710	8	410158	7	NULL	NULL	NULL	NULL	end of 14 days	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fractional rate of skeletal muscle protein synthesis and the whole body rate of protein breakdown were determined during a constant intravenous infusion of ( 13C ) leucine in 7 young ( 23 + / - 2 yr ; 86.2 + / - 4.6 kg ) healthy experienced male weight lifters before and at the end of 14 days of subcutaneous GH administration ( 40 microgram.kg-1 x day-1 ) .
	manualset3
156711	9	410158	7	NULL	NULL	0	NULL	subcutaneous GH administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The fractional rate of skeletal muscle protein synthesis and the whole body rate of protein breakdown were determined during a constant intravenous infusion of ( 13C ) leucine in 7 young ( 23 + / - 2 yr ; 86.2 + / - 4.6 kg ) healthy experienced male weight lifters before and at the end of 14 days of subcutaneous GH administration ( 40 microgram.kg-1 x day-1 ) .
	manualset3
157193	10	410158	7	NULL	NULL	0	NULL	 40 microgram.kg-1 x day-1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The fractional rate of skeletal muscle protein synthesis and the whole body rate of protein breakdown were determined during a constant intravenous infusion of ( 13C ) leucine in 7 young ( 23 + / - 2 yr ; 86.2 + / - 4.6 kg ) healthy experienced male weight lifters before and at the end of 14 days of subcutaneous GH administration ( 40 microgram.kg-1 x day-1 ) .
	manualset3
156712	1	410159	7	NULL	NULL	0	NULL	fractionation of cholesterol	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The fractionation of cholesterol in body fluids by means of solvent extraction .
	manualset3
156713	2	410159	7	NULL	NULL	0	NULL	body fluids	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The fractionation of cholesterol in body fluids by means of solvent extraction .
	manualset3
156714	3	410159	7	NULL	NULL	0	NULL	solvent extraction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The fractionation of cholesterol in body fluids by means of solvent extraction .
	manualset3
157324	4	410159	7	NULL	NULL	0	NULL	means	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The fractionation of cholesterol in body fluids by means of solvent extraction .
	manualset3
156715	1	410160	7	NULL	NULL	0	NULL	fracture displacement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The fracture displacement was initially 34 degrees .
	manualset3
156716	2	410160	7	NULL	NULL	0	NULL	34 degrees	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The fracture displacement was initially 34 degrees .
	manualset3
156717	1	410161	7	NULL	NULL	0	NULL	framework	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The framework is held together in part by strong N-H ... O hydrogen bonds between the imidazole NH groups of the L ligands and the carboxylate O atoms of 1 , 4-bdc dianions within different alpha-polonium nets .
	manualset3
156718	2	410161	7	NULL	NULL	0	NULL	strong N-H ... O hydrogen bonds	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The framework is held together in part by strong N-H ... O hydrogen bonds between the imidazole NH groups of the L ligands and the carboxylate O atoms of 1 , 4-bdc dianions within different alpha-polonium nets .
	manualset3
156719	3	410161	7	NULL	NULL	0	NULL	imidazole NH groups of the L ligands 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The framework is held together in part by strong N-H ... O hydrogen bonds between the imidazole NH groups of the L ligands and the carboxylate O atoms of 1 , 4-bdc dianions within different alpha-polonium nets .
	manualset3
156720	4	410161	7	NULL	NULL	0	NULL	carboxylate O atoms of 1 , 4-bdc dianions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The framework is held together in part by strong N-H ... O hydrogen bonds between the imidazole NH groups of the L ligands and the carboxylate O atoms of 1 , 4-bdc dianions within different alpha-polonium nets .
	manualset3
156721	5	410161	7	NULL	NULL	0	NULL	alpha-polonium nets	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The framework is held together in part by strong N-H ... O hydrogen bonds between the imidazole NH groups of the L ligands and the carboxylate O atoms of 1 , 4-bdc dianions within different alpha-polonium nets .
	manualset3
156722	1	410162	7	NULL	NULL	0	NULL	free , active insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The free , active insulin is extracted from the serum with a polyethylene glycol solution .
	manualset3
156723	2	410162	7	NULL	NULL	0	NULL	serum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The free , active insulin is extracted from the serum with a polyethylene glycol solution .
	manualset3
156724	3	410162	7	NULL	NULL	0	NULL	polyethylene glycol solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The free , active insulin is extracted from the serum with a polyethylene glycol solution .
	manualset3
156725	1	410163	7	NULL	NULL	0	NULL	free energy	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The free energy to close a TTTT end-loop is 2.12 kcal/mol ( 1 cal = 4.184 J ) .
	manualset3
156726	2	410163	7	NULL	NULL	0	NULL	 TTTT end-loop 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The free energy to close a TTTT end-loop is 2.12 kcal/mol ( 1 cal = 4.184 J ) .
	manualset3
156727	3	410163	7	NULL	NULL	0	NULL	2.12 kcal/mol	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The free energy to close a TTTT end-loop is 2.12 kcal/mol ( 1 cal = 4.184 J ) .
	manualset3
156728	4	410163	7	NULL	NULL	0	NULL	( 1 cal = 4.184 J )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The free energy to close a TTTT end-loop is 2.12 kcal/mol ( 1 cal = 4.184 J ) .
	manualset3
156729	1	410164	7	NULL	NULL	0	NULL	free lateral thoracic flap	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The free lateral thoracic flap has a longer vascular pedicle and larger-caliber vessels compared with the groin flap .
	manualset3
156730	2	410164	7	NULL	NULL	0	NULL	 longer vascular pedicle 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The free lateral thoracic flap has a longer vascular pedicle and larger-caliber vessels compared with the groin flap .
	manualset3
156731	3	410164	7	NULL	NULL	0	NULL	larger-caliber vessels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The free lateral thoracic flap has a longer vascular pedicle and larger-caliber vessels compared with the groin flap .
	manualset3
156732	4	410164	7	NULL	NULL	0	NULL	groin flap	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The free lateral thoracic flap has a longer vascular pedicle and larger-caliber vessels compared with the groin flap .
	manualset3
156733	1	410165	7	NULL	NULL	0	NULL	freezing mechanism of water	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The freezing mechanism of water contacted with mesoporous silicas with uniform pore shapes , both cylindrical and cagelike , was studied by thermodynamic and structural analyses with differential scanning calorimetry ( DSC ) and X-ray diffraction ( XRD ) together with adsorption measurements .
	manualset3
156734	2	410165	7	NULL	NULL	0	NULL	mesoporous silicas	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The freezing mechanism of water contacted with mesoporous silicas with uniform pore shapes , both cylindrical and cagelike , was studied by thermodynamic and structural analyses with differential scanning calorimetry ( DSC ) and X-ray diffraction ( XRD ) together with adsorption measurements .
	manualset3
156735	3	410165	7	NULL	NULL	0	NULL	uniform pore shapes	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The freezing mechanism of water contacted with mesoporous silicas with uniform pore shapes , both cylindrical and cagelike , was studied by thermodynamic and structural analyses with differential scanning calorimetry ( DSC ) and X-ray diffraction ( XRD ) together with adsorption measurements .
	manualset3
156736	4	410165	7	NULL	NULL	0	NULL	cylindrical and cagelike	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The freezing mechanism of water contacted with mesoporous silicas with uniform pore shapes , both cylindrical and cagelike , was studied by thermodynamic and structural analyses with differential scanning calorimetry ( DSC ) and X-ray diffraction ( XRD ) together with adsorption measurements .
	manualset3
156737	5	410165	7	NULL	NULL	0	NULL	thermodynamic analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The freezing mechanism of water contacted with mesoporous silicas with uniform pore shapes , both cylindrical and cagelike , was studied by thermodynamic and structural analyses with differential scanning calorimetry ( DSC ) and X-ray diffraction ( XRD ) together with adsorption measurements .
	manualset3
156738	6	410165	7	NULL	NULL	0	NULL	structural analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The freezing mechanism of water contacted with mesoporous silicas with uniform pore shapes , both cylindrical and cagelike , was studied by thermodynamic and structural analyses with differential scanning calorimetry ( DSC ) and X-ray diffraction ( XRD ) together with adsorption measurements .
	manualset3
156739	7	410165	7	NULL	NULL	0	NULL	differential scanning calorimetry ( DSC )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The freezing mechanism of water contacted with mesoporous silicas with uniform pore shapes , both cylindrical and cagelike , was studied by thermodynamic and structural analyses with differential scanning calorimetry ( DSC ) and X-ray diffraction ( XRD ) together with adsorption measurements .
	manualset3
156740	8	410165	7	NULL	NULL	0	NULL	X-ray diffraction ( XRD ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The freezing mechanism of water contacted with mesoporous silicas with uniform pore shapes , both cylindrical and cagelike , was studied by thermodynamic and structural analyses with differential scanning calorimetry ( DSC ) and X-ray diffraction ( XRD ) together with adsorption measurements .
	manualset3
156741	9	410165	7	NULL	NULL	0	NULL	adsorption measurements	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The freezing mechanism of water contacted with mesoporous silicas with uniform pore shapes , both cylindrical and cagelike , was studied by thermodynamic and structural analyses with differential scanning calorimetry ( DSC ) and X-ray diffraction ( XRD ) together with adsorption measurements .
	manualset3
156742	1	410166	7	NULL	NULL	0	NULL	survey	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey of enteric viruses and indicator bacteria was carried out in eight community water supply sources ( four wells and four springs ) in East Tennessee .
	manualset3
156743	2	410166	7	NULL	NULL	0	NULL	enteric viruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey of enteric viruses and indicator bacteria was carried out in eight community water supply sources ( four wells and four springs ) in East Tennessee .
	manualset3
156744	3	410166	7	NULL	NULL	0	NULL	indicator bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey of enteric viruses and indicator bacteria was carried out in eight community water supply sources ( four wells and four springs ) in East Tennessee .
	manualset3
156745	4	410166	7	NULL	NULL	0	NULL	eight community	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey of enteric viruses and indicator bacteria was carried out in eight community water supply sources ( four wells and four springs ) in East Tennessee .
	manualset3
156746	5	410166	7	NULL	NULL	NULL	NULL	water supply sources	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A survey of enteric viruses and indicator bacteria was carried out in eight community water supply sources ( four wells and four springs ) in East Tennessee .
	manualset3
156747	6	410166	7	NULL	NULL	0	NULL	four wells and four springs	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey of enteric viruses and indicator bacteria was carried out in eight community water supply sources ( four wells and four springs ) in East Tennessee .
	manualset3
156748	7	410166	7	NULL	NULL	0	NULL	East Tennessee	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey of enteric viruses and indicator bacteria was carried out in eight community water supply sources ( four wells and four springs ) in East Tennessee .
	manualset3
156750	1	410167	7	NULL	NULL	0	NULL	frequencies of MN	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequencies of MN in lymphocytes exposed to complex electromagnetic fields for 0 , 22 , 45 , 67 , and 89 min were 9.67 , 11.67 , 14.67 , 18.00 , and 20.33 per 1000 cells , respectively .
	manualset3
156751	2	410167	7	NULL	NULL	0	NULL	lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequencies of MN in lymphocytes exposed to complex electromagnetic fields for 0 , 22 , 45 , 67 , and 89 min were 9.67 , 11.67 , 14.67 , 18.00 , and 20.33 per 1000 cells , respectively .
	manualset3
156752	3	410167	7	NULL	NULL	0	NULL	complex electromagnetic fields	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequencies of MN in lymphocytes exposed to complex electromagnetic fields for 0 , 22 , 45 , 67 , and 89 min were 9.67 , 11.67 , 14.67 , 18.00 , and 20.33 per 1000 cells , respectively .
	manualset3
156753	4	410167	7	NULL	NULL	0	NULL	 0 , 22 , 45 , 67 , and 89 min	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequencies of MN in lymphocytes exposed to complex electromagnetic fields for 0 , 22 , 45 , 67 , and 89 min were 9.67 , 11.67 , 14.67 , 18.00 , and 20.33 per 1000 cells , respectively .
	manualset3
156754	5	410167	7	NULL	NULL	0	NULL	9.67 , 11.67 , 14.67 , 18.00 , and 20.33 per 1000 cells	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequencies of MN in lymphocytes exposed to complex electromagnetic fields for 0 , 22 , 45 , 67 , and 89 min were 9.67 , 11.67 , 14.67 , 18.00 , and 20.33 per 1000 cells , respectively .
	manualset3
156755	1	410168	7	NULL	NULL	0	NULL	 frequency A ( 0.20 )	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency A ( 0.20 ) of the A-allele was significantly lower among these Chinese controls than in the Caucasian control populations ( A = 0.54-0 .65 ) ( All P & lt ; 0.001 ) .
	manualset3
156756	2	410168	7	NULL	NULL	NULL	NULL	A-allele	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The frequency A ( 0.20 ) of the A-allele was significantly lower among these Chinese controls than in the Caucasian control populations ( A = 0.54-0 .65 ) ( All P & lt ; 0.001 ) .
	manualset3
156757	3	410168	7	NULL	NULL	0	NULL	Chinese controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency A ( 0.20 ) of the A-allele was significantly lower among these Chinese controls than in the Caucasian control populations ( A = 0.54-0 .65 ) ( All P & lt ; 0.001 ) .
	manualset3
156758	4	410168	7	NULL	NULL	0	NULL	Caucasian control populations 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency A ( 0.20 ) of the A-allele was significantly lower among these Chinese controls than in the Caucasian control populations ( A = 0.54-0 .65 ) ( All P & lt ; 0.001 ) .
	manualset3
156759	5	410168	7	NULL	NULL	0	NULL	( A = 0.54-0 .65 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency A ( 0.20 ) of the A-allele was significantly lower among these Chinese controls than in the Caucasian control populations ( A = 0.54-0 .65 ) ( All P & lt ; 0.001 ) .
	manualset3
156760	6	410168	7	NULL	NULL	0	NULL	( All P & lt ; 0.001 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency A ( 0.20 ) of the A-allele was significantly lower among these Chinese controls than in the Caucasian control populations ( A = 0.54-0 .65 ) ( All P & lt ; 0.001 ) .
	manualset3
156761	1	410169	7	NULL	NULL	NULL	NULL	frequency	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The frequency and amplitude of miniature endplate potentials ( MEPPs ) of the diaphragms obtained from mice injected intraperitoneally with purified IgG from MG patient were reduced by about 13 % and 20 % , respectively in comparison with results from normal mouse diaphragms .
	manualset3
156762	2	410169	7	NULL	NULL	NULL	NULL	amplitude	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The frequency and amplitude of miniature endplate potentials ( MEPPs ) of the diaphragms obtained from mice injected intraperitoneally with purified IgG from MG patient were reduced by about 13 % and 20 % , respectively in comparison with results from normal mouse diaphragms .
	manualset3
156763	3	410169	7	NULL	NULL	0	NULL	miniature endplate potentials ( MEPPs )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency and amplitude of miniature endplate potentials ( MEPPs ) of the diaphragms obtained from mice injected intraperitoneally with purified IgG from MG patient were reduced by about 13 % and 20 % , respectively in comparison with results from normal mouse diaphragms .
	manualset3
156764	4	410169	7	NULL	NULL	0	NULL	 diaphragms	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency and amplitude of miniature endplate potentials ( MEPPs ) of the diaphragms obtained from mice injected intraperitoneally with purified IgG from MG patient were reduced by about 13 % and 20 % , respectively in comparison with results from normal mouse diaphragms .
	manualset3
156765	5	410169	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency and amplitude of miniature endplate potentials ( MEPPs ) of the diaphragms obtained from mice injected intraperitoneally with purified IgG from MG patient were reduced by about 13 % and 20 % , respectively in comparison with results from normal mouse diaphragms .
	manualset3
156766	6	410169	7	NULL	NULL	0	NULL	purified IgG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency and amplitude of miniature endplate potentials ( MEPPs ) of the diaphragms obtained from mice injected intraperitoneally with purified IgG from MG patient were reduced by about 13 % and 20 % , respectively in comparison with results from normal mouse diaphragms .
	manualset3
156767	7	410169	7	NULL	NULL	0	NULL	MG patient	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency and amplitude of miniature endplate potentials ( MEPPs ) of the diaphragms obtained from mice injected intraperitoneally with purified IgG from MG patient were reduced by about 13 % and 20 % , respectively in comparison with results from normal mouse diaphragms .
	manualset3
156768	8	410169	7	NULL	NULL	0	NULL	13 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency and amplitude of miniature endplate potentials ( MEPPs ) of the diaphragms obtained from mice injected intraperitoneally with purified IgG from MG patient were reduced by about 13 % and 20 % , respectively in comparison with results from normal mouse diaphragms .
	manualset3
156769	9	410169	7	NULL	NULL	0	NULL	20 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency and amplitude of miniature endplate potentials ( MEPPs ) of the diaphragms obtained from mice injected intraperitoneally with purified IgG from MG patient were reduced by about 13 % and 20 % , respectively in comparison with results from normal mouse diaphragms .
	manualset3
156770	10	410169	7	NULL	NULL	0	NULL	results	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency and amplitude of miniature endplate potentials ( MEPPs ) of the diaphragms obtained from mice injected intraperitoneally with purified IgG from MG patient were reduced by about 13 % and 20 % , respectively in comparison with results from normal mouse diaphragms .
	manualset3
156771	11	410169	7	NULL	NULL	0	NULL	normal mouse diaphragms	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency and amplitude of miniature endplate potentials ( MEPPs ) of the diaphragms obtained from mice injected intraperitoneally with purified IgG from MG patient were reduced by about 13 % and 20 % , respectively in comparison with results from normal mouse diaphragms .
	manualset3
156772	1	410170	7	NULL	NULL	0	NULL	frequency of CD34 ( + ) cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of CD34 ( + ) cells was higher in Wnt-expressing cocultures and cellular morphology indicated that coculture in the presence of Wnt genes resulted in higher numbers of less differentiated hematopoietic cells and fewer mature cells than controls .
	manualset3
156773	2	410170	7	NULL	NULL	NULL	NULL	Wnt-expressing cocultures	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The frequency of CD34 ( + ) cells was higher in Wnt-expressing cocultures and cellular morphology indicated that coculture in the presence of Wnt genes resulted in higher numbers of less differentiated hematopoietic cells and fewer mature cells than controls .
	manualset3
156774	3	410170	7	NULL	NULL	0	NULL	cellular morphology	AnatomicalPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of CD34 ( + ) cells was higher in Wnt-expressing cocultures and cellular morphology indicated that coculture in the presence of Wnt genes resulted in higher numbers of less differentiated hematopoietic cells and fewer mature cells than controls .
	manualset3
156775	4	410170	7	NULL	NULL	0	NULL	coculture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of CD34 ( + ) cells was higher in Wnt-expressing cocultures and cellular morphology indicated that coculture in the presence of Wnt genes resulted in higher numbers of less differentiated hematopoietic cells and fewer mature cells than controls .
	manualset3
156776	5	410170	7	NULL	NULL	0	NULL	Wnt genes 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of CD34 ( + ) cells was higher in Wnt-expressing cocultures and cellular morphology indicated that coculture in the presence of Wnt genes resulted in higher numbers of less differentiated hematopoietic cells and fewer mature cells than controls .
	manualset3
156777	6	410170	7	NULL	NULL	0	NULL	less differentiated hematopoietic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of CD34 ( + ) cells was higher in Wnt-expressing cocultures and cellular morphology indicated that coculture in the presence of Wnt genes resulted in higher numbers of less differentiated hematopoietic cells and fewer mature cells than controls .
	manualset3
156778	7	410170	7	NULL	NULL	0	NULL	mature cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of CD34 ( + ) cells was higher in Wnt-expressing cocultures and cellular morphology indicated that coculture in the presence of Wnt genes resulted in higher numbers of less differentiated hematopoietic cells and fewer mature cells than controls .
	manualset3
156779	8	410170	7	NULL	NULL	0	NULL	controls	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of CD34 ( + ) cells was higher in Wnt-expressing cocultures and cellular morphology indicated that coculture in the presence of Wnt genes resulted in higher numbers of less differentiated hematopoietic cells and fewer mature cells than controls .
	manualset3
157325	9	410170	7	NULL	NULL	0	NULL	higher numbers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of CD34 ( + ) cells was higher in Wnt-expressing cocultures and cellular morphology indicated that coculture in the presence of Wnt genes resulted in higher numbers of less differentiated hematopoietic cells and fewer mature cells than controls .
	manualset3
156780	1	410171	7	NULL	NULL	NULL	NULL	 HLA-B42	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The frequency of HLA-B42 was significantly ( P = 0.002 ) increased in recipients who rejected the graft .
	manualset3
156781	2	410171	7	NULL	NULL	0	NULL	( P = 0.002 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of HLA-B42 was significantly ( P = 0.002 ) increased in recipients who rejected the graft .
	manualset3
156782	3	410171	7	NULL	NULL	0	NULL	recipients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of HLA-B42 was significantly ( P = 0.002 ) increased in recipients who rejected the graft .
	manualset3
156783	4	410171	7	NULL	NULL	0	NULL	graft	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of HLA-B42 was significantly ( P = 0.002 ) increased in recipients who rejected the graft .
	manualset3
157326	5	410171	7	NULL	NULL	0	NULL	frequency	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of HLA-B42 was significantly ( P = 0.002 ) increased in recipients who rejected the graft .
	manualset3
156784	1	410172	7	NULL	NULL	NULL	NULL	 Johne 's disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The frequency of Johne 's disease in cattle in south west England was estimated from data collected by telephone interviews with veterinarians and farmers .
	manualset3
156785	2	410172	7	NULL	NULL	0	NULL	cattle	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of Johne 's disease in cattle in south west England was estimated from data collected by telephone interviews with veterinarians and farmers .
	manualset3
156786	3	410172	7	NULL	NULL	0	NULL	south west England	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of Johne 's disease in cattle in south west England was estimated from data collected by telephone interviews with veterinarians and farmers .
	manualset3
156787	4	410172	7	NULL	NULL	0	NULL	telephone interviews	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of Johne 's disease in cattle in south west England was estimated from data collected by telephone interviews with veterinarians and farmers .
	manualset3
156788	5	410172	7	NULL	NULL	0	NULL	veterinarians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of Johne 's disease in cattle in south west England was estimated from data collected by telephone interviews with veterinarians and farmers .
	manualset3
156789	6	410172	7	NULL	NULL	0	NULL	farmers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of Johne 's disease in cattle in south west England was estimated from data collected by telephone interviews with veterinarians and farmers .
	manualset3
157194	7	410172	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of Johne 's disease in cattle in south west England was estimated from data collected by telephone interviews with veterinarians and farmers .
	manualset3
157327	8	410172	7	NULL	NULL	0	NULL	 frequency	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of Johne 's disease in cattle in south west England was estimated from data collected by telephone interviews with veterinarians and farmers .
	manualset3
156790	1	410173	7	NULL	NULL	0	NULL	frequency of documentation	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of documentation of depressive signs and symptoms after the screening procedure with the short GDS was associated with subsequent prescription of antidepressants and referral to the psychogeriatric service .
	manualset3
156791	2	410173	7	NULL	NULL	0	NULL	depressive signs 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of documentation of depressive signs and symptoms after the screening procedure with the short GDS was associated with subsequent prescription of antidepressants and referral to the psychogeriatric service .
	manualset3
156792	3	410173	7	NULL	NULL	0	NULL	symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of documentation of depressive signs and symptoms after the screening procedure with the short GDS was associated with subsequent prescription of antidepressants and referral to the psychogeriatric service .
	manualset3
156793	4	410173	7	NULL	NULL	0	NULL	screening procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of documentation of depressive signs and symptoms after the screening procedure with the short GDS was associated with subsequent prescription of antidepressants and referral to the psychogeriatric service .
	manualset3
156794	5	410173	7	NULL	NULL	0	NULL	short GDS	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of documentation of depressive signs and symptoms after the screening procedure with the short GDS was associated with subsequent prescription of antidepressants and referral to the psychogeriatric service .
	manualset3
156795	6	410173	7	NULL	NULL	0	NULL	 prescription 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of documentation of depressive signs and symptoms after the screening procedure with the short GDS was associated with subsequent prescription of antidepressants and referral to the psychogeriatric service .
	manualset3
156796	7	410173	7	NULL	NULL	0	NULL	antidepressants	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of documentation of depressive signs and symptoms after the screening procedure with the short GDS was associated with subsequent prescription of antidepressants and referral to the psychogeriatric service .
	manualset3
156797	8	410173	7	NULL	NULL	0	NULL	psychogeriatric service	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of documentation of depressive signs and symptoms after the screening procedure with the short GDS was associated with subsequent prescription of antidepressants and referral to the psychogeriatric service .
	manualset3
157328	9	410173	7	NULL	NULL	0	NULL	referral	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of documentation of depressive signs and symptoms after the screening procedure with the short GDS was associated with subsequent prescription of antidepressants and referral to the psychogeriatric service .
	manualset3
156798	1	410174	7	NULL	NULL	0	NULL	frequency of endophytic fungi 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of endophytic fungi mainly depended on the size of the island , explaining 32-35 % of the variation , and the distance to the mainland explaining 29-35 % of the variation .
	manualset3
156799	2	410174	7	NULL	NULL	NULL	NULL	size of the island	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The frequency of endophytic fungi mainly depended on the size of the island , explaining 32-35 % of the variation , and the distance to the mainland explaining 29-35 % of the variation .
	manualset3
156800	3	410174	7	NULL	NULL	0	NULL	32-35 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of endophytic fungi mainly depended on the size of the island , explaining 32-35 % of the variation , and the distance to the mainland explaining 29-35 % of the variation .
	manualset3
156801	4	410174	7	NULL	NULL	0	NULL	variation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of endophytic fungi mainly depended on the size of the island , explaining 32-35 % of the variation , and the distance to the mainland explaining 29-35 % of the variation .
	manualset3
156802	5	410174	7	NULL	NULL	0	NULL	distance	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of endophytic fungi mainly depended on the size of the island , explaining 32-35 % of the variation , and the distance to the mainland explaining 29-35 % of the variation .
	manualset3
156803	6	410174	7	NULL	NULL	0	NULL	mainland	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of endophytic fungi mainly depended on the size of the island , explaining 32-35 % of the variation , and the distance to the mainland explaining 29-35 % of the variation .
	manualset3
156804	7	410174	7	NULL	NULL	0	NULL	29-35 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of endophytic fungi mainly depended on the size of the island , explaining 32-35 % of the variation , and the distance to the mainland explaining 29-35 % of the variation .
	manualset3
156805	8	410174	7	NULL	NULL	0	NULL	variation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of endophytic fungi mainly depended on the size of the island , explaining 32-35 % of the variation , and the distance to the mainland explaining 29-35 % of the variation .
	manualset3
156806	1	410175	7	NULL	NULL	0	NULL	frequency of smokers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of smokers was significantly greater in the HDRU than in the other three groups studied .
	manualset3
156807	2	410175	7	NULL	NULL	0	NULL	HDRU	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of smokers was significantly greater in the HDRU than in the other three groups studied .
	manualset3
156808	3	410175	7	NULL	NULL	0	NULL	three groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of smokers was significantly greater in the HDRU than in the other three groups studied .
	manualset3
156809	1	410176	7	NULL	NULL	0	NULL	survey	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey of inpatient alcoholics in Japan .
	manualset3
156810	2	410176	7	NULL	NULL	NULL	NULL	inpatient alcoholics	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A survey of inpatient alcoholics in Japan .
	manualset3
156811	3	410176	7	NULL	NULL	0	NULL	Japan	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey of inpatient alcoholics in Japan .
	manualset3
156812	1	410177	7	NULL	NULL	0	NULL	frequency of spermatozoa	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of spermatozoa with two chromosome 7 signals was 6.4 + / - 3.9 / 10 , 000 .
	manualset3
156813	2	410177	7	NULL	NULL	NULL	NULL	two chromosome 7 signals	Chromosome												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The frequency of spermatozoa with two chromosome 7 signals was 6.4 + / - 3.9 / 10 , 000 .
	manualset3
156815	3	410177	7	NULL	NULL	NULL	NULL	6.4 + / - 3.9 / 10 , 000 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The frequency of spermatozoa with two chromosome 7 signals was 6.4 + / - 3.9 / 10 , 000 .
	manualset3
156816	1	410178	7	NULL	NULL	0	NULL	frequency of the haplotype	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of the haplotype HLA-Bw44 , - DR5 was 0.133 compared with 0.007 ( X2 = 27.04 , P less than 10 ( -6 ) and for HLA-Bw35 , - Cw4 , - DR5 , it was 0.093 compared with 0.11 ( X2 = 13.83 , P = 0.0002 ) .
	manualset3
156817	2	410178	7	NULL	NULL	0	NULL	HLA-Bw44	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of the haplotype HLA-Bw44 , - DR5 was 0.133 compared with 0.007 ( X2 = 27.04 , P less than 10 ( -6 ) and for HLA-Bw35 , - Cw4 , - DR5 , it was 0.093 compared with 0.11 ( X2 = 13.83 , P = 0.0002 ) .
	manualset3
156818	3	410178	7	NULL	NULL	0	NULL	- DR5	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of the haplotype HLA-Bw44 , - DR5 was 0.133 compared with 0.007 ( X2 = 27.04 , P less than 10 ( -6 ) and for HLA-Bw35 , - Cw4 , - DR5 , it was 0.093 compared with 0.11 ( X2 = 13.83 , P = 0.0002 ) .
	manualset3
156819	4	410178	7	NULL	NULL	0	NULL	0.133	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of the haplotype HLA-Bw44 , - DR5 was 0.133 compared with 0.007 ( X2 = 27.04 , P less than 10 ( -6 ) and for HLA-Bw35 , - Cw4 , - DR5 , it was 0.093 compared with 0.11 ( X2 = 13.83 , P = 0.0002 ) .
	manualset3
156820	5	410178	7	NULL	NULL	0	NULL	0.007	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of the haplotype HLA-Bw44 , - DR5 was 0.133 compared with 0.007 ( X2 = 27.04 , P less than 10 ( -6 ) and for HLA-Bw35 , - Cw4 , - DR5 , it was 0.093 compared with 0.11 ( X2 = 13.83 , P = 0.0002 ) .
	manualset3
156821	6	410178	7	NULL	NULL	0	NULL	( X2 = 27.04 , P less than 10 ( -6 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of the haplotype HLA-Bw44 , - DR5 was 0.133 compared with 0.007 ( X2 = 27.04 , P less than 10 ( -6 ) and for HLA-Bw35 , - Cw4 , - DR5 , it was 0.093 compared with 0.11 ( X2 = 13.83 , P = 0.0002 ) .
	manualset3
156822	7	410178	7	NULL	NULL	0	NULL	HLA-Bw35	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of the haplotype HLA-Bw44 , - DR5 was 0.133 compared with 0.007 ( X2 = 27.04 , P less than 10 ( -6 ) and for HLA-Bw35 , - Cw4 , - DR5 , it was 0.093 compared with 0.11 ( X2 = 13.83 , P = 0.0002 ) .
	manualset3
156823	8	410178	7	NULL	NULL	0	NULL	- Cw4	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of the haplotype HLA-Bw44 , - DR5 was 0.133 compared with 0.007 ( X2 = 27.04 , P less than 10 ( -6 ) and for HLA-Bw35 , - Cw4 , - DR5 , it was 0.093 compared with 0.11 ( X2 = 13.83 , P = 0.0002 ) .
	manualset3
156824	9	410178	7	NULL	NULL	0	NULL	- DR5	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of the haplotype HLA-Bw44 , - DR5 was 0.133 compared with 0.007 ( X2 = 27.04 , P less than 10 ( -6 ) and for HLA-Bw35 , - Cw4 , - DR5 , it was 0.093 compared with 0.11 ( X2 = 13.83 , P = 0.0002 ) .
	manualset3
156825	10	410178	7	NULL	NULL	0	NULL	0.093	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of the haplotype HLA-Bw44 , - DR5 was 0.133 compared with 0.007 ( X2 = 27.04 , P less than 10 ( -6 ) and for HLA-Bw35 , - Cw4 , - DR5 , it was 0.093 compared with 0.11 ( X2 = 13.83 , P = 0.0002 ) .
	manualset3
156826	11	410178	7	NULL	NULL	0	NULL	0.11	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of the haplotype HLA-Bw44 , - DR5 was 0.133 compared with 0.007 ( X2 = 27.04 , P less than 10 ( -6 ) and for HLA-Bw35 , - Cw4 , - DR5 , it was 0.093 compared with 0.11 ( X2 = 13.83 , P = 0.0002 ) .
	manualset3
156827	12	410178	7	NULL	NULL	0	NULL	( X2 = 13.83 , P = 0.0002 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of the haplotype HLA-Bw44 , - DR5 was 0.133 compared with 0.007 ( X2 = 27.04 , P less than 10 ( -6 ) and for HLA-Bw35 , - Cw4 , - DR5 , it was 0.093 compared with 0.11 ( X2 = 13.83 , P = 0.0002 ) .
	manualset3
156828	1	410179	7	NULL	NULL	0	NULL	frequency of the oscillation	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of the oscillation did vary with different odorant compounds in both olfactory epithelium and bulb ( OE and OB ) : amyl acetate , ethyl fenchol and d-carvone elicited oscillations of significantly different frequencies , and there was no difference in OE and OB oscillation frequencies .
	manualset3
156829	2	410179	7	NULL	NULL	0	NULL	different odorant compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of the oscillation did vary with different odorant compounds in both olfactory epithelium and bulb ( OE and OB ) : amyl acetate , ethyl fenchol and d-carvone elicited oscillations of significantly different frequencies , and there was no difference in OE and OB oscillation frequencies .
	manualset3
156830	4	410179	7	NULL	NULL	NULL	NULL	amyl acetate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The frequency of the oscillation did vary with different odorant compounds in both olfactory epithelium and bulb ( OE and OB ) : amyl acetate , ethyl fenchol and d-carvone elicited oscillations of significantly different frequencies , and there was no difference in OE and OB oscillation frequencies .
	manualset3
156831	5	410179	7	NULL	NULL	0	NULL	ethyl fenchol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of the oscillation did vary with different odorant compounds in both olfactory epithelium and bulb ( OE and OB ) : amyl acetate , ethyl fenchol and d-carvone elicited oscillations of significantly different frequencies , and there was no difference in OE and OB oscillation frequencies .
	manualset3
156832	3	410179	7	NULL	NULL	0	NULL	olfactory epithelium and bulb ( OE and OB )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of the oscillation did vary with different odorant compounds in both olfactory epithelium and bulb ( OE and OB ) : amyl acetate , ethyl fenchol and d-carvone elicited oscillations of significantly different frequencies , and there was no difference in OE and OB oscillation frequencies .
	manualset3
156833	6	410179	7	NULL	NULL	0	NULL	d-carvone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of the oscillation did vary with different odorant compounds in both olfactory epithelium and bulb ( OE and OB ) : amyl acetate , ethyl fenchol and d-carvone elicited oscillations of significantly different frequencies , and there was no difference in OE and OB oscillation frequencies .
	manualset3
156834	7	410179	7	NULL	NULL	0	NULL	oscillations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of the oscillation did vary with different odorant compounds in both olfactory epithelium and bulb ( OE and OB ) : amyl acetate , ethyl fenchol and d-carvone elicited oscillations of significantly different frequencies , and there was no difference in OE and OB oscillation frequencies .
	manualset3
156835	8	410179	7	NULL	NULL	NULL	NULL	OE and OB oscillation frequencies	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The frequency of the oscillation did vary with different odorant compounds in both olfactory epithelium and bulb ( OE and OB ) : amyl acetate , ethyl fenchol and d-carvone elicited oscillations of significantly different frequencies , and there was no difference in OE and OB oscillation frequencies .
	manualset3
157493	9	410179	7	NULL	NULL	0	NULL	 frequencies	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of the oscillation did vary with different odorant compounds in both olfactory epithelium and bulb ( OE and OB ) : amyl acetate , ethyl fenchol and d-carvone elicited oscillations of significantly different frequencies , and there was no difference in OE and OB oscillation frequencies .
	manualset3
157494	10	410179	7	NULL	NULL	0	NULL	difference 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of the oscillation did vary with different odorant compounds in both olfactory epithelium and bulb ( OE and OB ) : amyl acetate , ethyl fenchol and d-carvone elicited oscillations of significantly different frequencies , and there was no difference in OE and OB oscillation frequencies .
	manualset3
156836	1	410180	7	NULL	NULL	0	NULL	frequency of total severe hypoglycemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of total severe hypoglycemia was significantly decreased in the low-SUITO group compared to pretransplant status and further decreased in the middle - and high-SUITO group .
	manualset3
156837	2	410180	7	NULL	NULL	0	NULL	low-SUITO group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of total severe hypoglycemia was significantly decreased in the low-SUITO group compared to pretransplant status and further decreased in the middle - and high-SUITO group .
	manualset3
156838	3	410180	7	NULL	NULL	0	NULL	pretransplant status	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of total severe hypoglycemia was significantly decreased in the low-SUITO group compared to pretransplant status and further decreased in the middle - and high-SUITO group .
	manualset3
156839	4	410180	7	NULL	NULL	0	NULL	middle-SUITO group 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of total severe hypoglycemia was significantly decreased in the low-SUITO group compared to pretransplant status and further decreased in the middle - and high-SUITO group .
	manualset3
156840	5	410180	7	NULL	NULL	0	NULL	high-SUITO group 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of total severe hypoglycemia was significantly decreased in the low-SUITO group compared to pretransplant status and further decreased in the middle - and high-SUITO group .
	manualset3
156841	1	410181	7	NULL	NULL	0	NULL	front-tracking approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The front-tracking approach illustrated is of relevance in the development of detailed and accurate models of drug delivery from swellable cylindrical matrices involving both axial and radial diffusion .
	manualset3
156842	2	410181	7	NULL	NULL	0	NULL	accurate models	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The front-tracking approach illustrated is of relevance in the development of detailed and accurate models of drug delivery from swellable cylindrical matrices involving both axial and radial diffusion .
	manualset3
156843	3	410181	7	NULL	NULL	0	NULL	drug delivery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The front-tracking approach illustrated is of relevance in the development of detailed and accurate models of drug delivery from swellable cylindrical matrices involving both axial and radial diffusion .
	manualset3
156844	4	410181	7	NULL	NULL	0	NULL	swellable cylindrical matrices	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The front-tracking approach illustrated is of relevance in the development of detailed and accurate models of drug delivery from swellable cylindrical matrices involving both axial and radial diffusion .
	manualset3
156845	5	410181	7	NULL	NULL	0	NULL	axial and radial diffusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The front-tracking approach illustrated is of relevance in the development of detailed and accurate models of drug delivery from swellable cylindrical matrices involving both axial and radial diffusion .
	manualset3
157330	6	410181	7	NULL	NULL	NULL	NULL	development	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The front-tracking approach illustrated is of relevance in the development of detailed and accurate models of drug delivery from swellable cylindrical matrices involving both axial and radial diffusion .
	manualset3
157495	7	410181	7	NULL	NULL	0	NULL	 relevance	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The front-tracking approach illustrated is of relevance in the development of detailed and accurate models of drug delivery from swellable cylindrical matrices involving both axial and radial diffusion .
	manualset3
156846	1	410182	7	NULL	NULL	0	NULL	fruit body	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The fruit body and in particular the gleba development of several species of Lycoperdaceae has been examined by light microscopic analysis of microtome sections of fruit body primordia in different ontogenetic stages .
	manualset3
156847	2	410182	7	NULL	NULL	0	NULL	gleba development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The fruit body and in particular the gleba development of several species of Lycoperdaceae has been examined by light microscopic analysis of microtome sections of fruit body primordia in different ontogenetic stages .
	manualset3
156848	3	410182	7	NULL	NULL	0	NULL	several species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The fruit body and in particular the gleba development of several species of Lycoperdaceae has been examined by light microscopic analysis of microtome sections of fruit body primordia in different ontogenetic stages .
	manualset3
156849	4	410182	7	NULL	NULL	NULL	NULL	Lycoperdaceae	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fruit body and in particular the gleba development of several species of Lycoperdaceae has been examined by light microscopic analysis of microtome sections of fruit body primordia in different ontogenetic stages .
	manualset3
156850	5	410182	7	NULL	NULL	0	NULL	light microscopic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The fruit body and in particular the gleba development of several species of Lycoperdaceae has been examined by light microscopic analysis of microtome sections of fruit body primordia in different ontogenetic stages .
	manualset3
156851	6	410182	7	NULL	NULL	0	NULL	microtome sections of fruit body primordia	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The fruit body and in particular the gleba development of several species of Lycoperdaceae has been examined by light microscopic analysis of microtome sections of fruit body primordia in different ontogenetic stages .
	manualset3
156852	7	410182	7	NULL	NULL	0	NULL	ontogenetic stages	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The fruit body and in particular the gleba development of several species of Lycoperdaceae has been examined by light microscopic analysis of microtome sections of fruit body primordia in different ontogenetic stages .
	manualset3
156853	1	410183	7	NULL	NULL	0	NULL	ftsZ17 ( Spo ) allele	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The ftsZ17 ( Spo ) allele gave rise to a classical white phenotype .
	manualset3
156854	2	410183	7	NULL	NULL	NULL	NULL	classical white phenotype	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ftsZ17 ( Spo ) allele gave rise to a classical white phenotype .
	manualset3
156855	1	410184	7	NULL	NULL	0	NULL	full-size human SURF-6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The full-size human SURF-6 was expressed as a recombinant GST-fusion protein and used as an antigen to generate monoclonal antibodies , S79 and S148 , specific for SURF-6 .
	manualset3
156856	2	410184	7	NULL	NULL	0	NULL	 recombinant GST-fusion protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The full-size human SURF-6 was expressed as a recombinant GST-fusion protein and used as an antigen to generate monoclonal antibodies , S79 and S148 , specific for SURF-6 .
	manualset3
156857	3	410184	7	NULL	NULL	0	NULL	antigen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The full-size human SURF-6 was expressed as a recombinant GST-fusion protein and used as an antigen to generate monoclonal antibodies , S79 and S148 , specific for SURF-6 .
	manualset3
156858	4	410184	7	NULL	NULL	0	NULL	monoclonal antibodies 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The full-size human SURF-6 was expressed as a recombinant GST-fusion protein and used as an antigen to generate monoclonal antibodies , S79 and S148 , specific for SURF-6 .
	manualset3
156859	5	410184	7	NULL	NULL	0	NULL	S79	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The full-size human SURF-6 was expressed as a recombinant GST-fusion protein and used as an antigen to generate monoclonal antibodies , S79 and S148 , specific for SURF-6 .
	manualset3
156860	6	410184	7	NULL	NULL	0	NULL	S148	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The full-size human SURF-6 was expressed as a recombinant GST-fusion protein and used as an antigen to generate monoclonal antibodies , S79 and S148 , specific for SURF-6 .
	manualset3
156861	7	410184	7	NULL	NULL	0	NULL	SURF-6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The full-size human SURF-6 was expressed as a recombinant GST-fusion protein and used as an antigen to generate monoclonal antibodies , S79 and S148 , specific for SURF-6 .
	manualset3
156862	1	410185	7	NULL	NULL	0	NULL	full length GAPDH protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The full length GAPDH protein was subsequently expressed in E. coli , purified as His-tag protein and confirmed to be catalytically active .
	manualset3
156863	2	410185	7	NULL	NULL	0	NULL	E. coli 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The full length GAPDH protein was subsequently expressed in E. coli , purified as His-tag protein and confirmed to be catalytically active .
	manualset3
156864	3	410185	7	NULL	NULL	0	NULL	 His-tag protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The full length GAPDH protein was subsequently expressed in E. coli , purified as His-tag protein and confirmed to be catalytically active .
	manualset3
156880	1	410186	7	NULL	NULL	0	NULL	full length of the cDNAs	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The full length of the cDNAs for ER , ER1 , and ER2 were isolated and characterized from Gobiocypris rarus .
	manualset3
156881	2	410186	7	NULL	NULL	0	NULL	ER 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The full length of the cDNAs for ER , ER1 , and ER2 were isolated and characterized from Gobiocypris rarus .
	manualset3
156882	3	410186	7	NULL	NULL	0	NULL	ER1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The full length of the cDNAs for ER , ER1 , and ER2 were isolated and characterized from Gobiocypris rarus .
	manualset3
156883	4	410186	7	NULL	NULL	0	NULL	ER2	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The full length of the cDNAs for ER , ER1 , and ER2 were isolated and characterized from Gobiocypris rarus .
	manualset3
156884	5	410186	7	NULL	NULL	0	NULL	Gobiocypris rarus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The full length of the cDNAs for ER , ER1 , and ER2 were isolated and characterized from Gobiocypris rarus .
	manualset3
156885	1	410187	7	NULL	NULL	NULL	NULL	 function 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The function of 111In-labelled platelets has been assessed by collagen-induced aggregation of platelets in samples of whole blood .
	manualset3
156887	2	410187	7	NULL	NULL	0	NULL	111In-labelled platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The function of 111In-labelled platelets has been assessed by collagen-induced aggregation of platelets in samples of whole blood .
	manualset3
156888	3	410187	7	NULL	NULL	0	NULL	collagen-induced aggregation of platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The function of 111In-labelled platelets has been assessed by collagen-induced aggregation of platelets in samples of whole blood .
	manualset3
156889	4	410187	7	NULL	NULL	0	NULL	whole blood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The function of 111In-labelled platelets has been assessed by collagen-induced aggregation of platelets in samples of whole blood .
	manualset3
156890	1	410188	7	NULL	NULL	0	NULL	function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The function of AtDCL2 and other DCLs has been much studied but little has been done to characterize the DCLs transcripts before they are translated into proteins .
	manualset3
156891	2	410188	7	NULL	NULL	0	NULL	AtDCL2	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The function of AtDCL2 and other DCLs has been much studied but little has been done to characterize the DCLs transcripts before they are translated into proteins .
	manualset3
156892	3	410188	7	NULL	NULL	0	NULL	DCLs	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The function of AtDCL2 and other DCLs has been much studied but little has been done to characterize the DCLs transcripts before they are translated into proteins .
	manualset3
156893	4	410188	7	NULL	NULL	0	NULL	DCLs transcripts	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The function of AtDCL2 and other DCLs has been much studied but little has been done to characterize the DCLs transcripts before they are translated into proteins .
	manualset3
156894	5	410188	7	NULL	NULL	0	NULL	proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The function of AtDCL2 and other DCLs has been much studied but little has been done to characterize the DCLs transcripts before they are translated into proteins .
	manualset3
156895	1	410189	7	NULL	NULL	0	NULL	 function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The function of CRFR2 , in particular , has remained elusive despite its presence in both the CNS and periphery .
	manualset3
156896	2	410189	7	NULL	NULL	0	NULL	CRFR2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The function of CRFR2 , in particular , has remained elusive despite its presence in both the CNS and periphery .
	manualset3
156897	3	410189	7	NULL	NULL	0	NULL	CNS	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The function of CRFR2 , in particular , has remained elusive despite its presence in both the CNS and periphery .
	manualset3
156898	4	410189	7	NULL	NULL	0	NULL	periphery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The function of CRFR2 , in particular , has remained elusive despite its presence in both the CNS and periphery .
	manualset3
157331	5	410189	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The function of CRFR2 , in particular , has remained elusive despite its presence in both the CNS and periphery .
	manualset3
156899	1	410190	7	NULL	NULL	0	NULL	function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The function of guanine nucleotide binding ( G ) proteins is Mg ( 2 + ) dependent with guanine nucleotide exchange requiring higher metal ion concentration than guanosine 5 ' - triphosphate hydrolysis .
	manualset3
156900	2	410190	7	NULL	NULL	0	NULL	guanine nucleotide binding ( G ) proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The function of guanine nucleotide binding ( G ) proteins is Mg ( 2 + ) dependent with guanine nucleotide exchange requiring higher metal ion concentration than guanosine 5 ' - triphosphate hydrolysis .
	manualset3
156901	3	410190	7	NULL	NULL	0	NULL	Mg ( 2 + ) dependent with guanine nucleotide exchange	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The function of guanine nucleotide binding ( G ) proteins is Mg ( 2 + ) dependent with guanine nucleotide exchange requiring higher metal ion concentration than guanosine 5 ' - triphosphate hydrolysis .
	manualset3
156902	4	410190	7	NULL	NULL	0	NULL	higher metal ion concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The function of guanine nucleotide binding ( G ) proteins is Mg ( 2 + ) dependent with guanine nucleotide exchange requiring higher metal ion concentration than guanosine 5 ' - triphosphate hydrolysis .
	manualset3
156903	5	410190	7	NULL	NULL	NULL	NULL	guanosine 5 ' - triphosphate hydrolysis	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The function of guanine nucleotide binding ( G ) proteins is Mg ( 2 + ) dependent with guanine nucleotide exchange requiring higher metal ion concentration than guanosine 5 ' - triphosphate hydrolysis .
	manualset3
156905	1	410191	7	NULL	NULL	0	NULL	 function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The function of the neuronal isoform of nitric oxide synthase ( nNOS ) was studied by comparing the effects of the specific nNOS blocker 7-nitro indazole monosodium salt ( 7-NINA ) with that of the general NOS inhibitor N ( G ) - nitro-L-arginine ( L-NA ) in isolated rat basilar arteries ( BAs ) .
	manualset3
156906	2	410191	7	NULL	NULL	0	NULL	neuronal isoform of nitric oxide synthase ( nNOS )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The function of the neuronal isoform of nitric oxide synthase ( nNOS ) was studied by comparing the effects of the specific nNOS blocker 7-nitro indazole monosodium salt ( 7-NINA ) with that of the general NOS inhibitor N ( G ) - nitro-L-arginine ( L-NA ) in isolated rat basilar arteries ( BAs ) .
	manualset3
156907	3	410191	7	NULL	NULL	0	NULL	specific nNOS blocker 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The function of the neuronal isoform of nitric oxide synthase ( nNOS ) was studied by comparing the effects of the specific nNOS blocker 7-nitro indazole monosodium salt ( 7-NINA ) with that of the general NOS inhibitor N ( G ) - nitro-L-arginine ( L-NA ) in isolated rat basilar arteries ( BAs ) .
	manualset3
156908	4	410191	7	NULL	NULL	0	NULL	7-nitro indazole monosodium salt ( 7-NINA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The function of the neuronal isoform of nitric oxide synthase ( nNOS ) was studied by comparing the effects of the specific nNOS blocker 7-nitro indazole monosodium salt ( 7-NINA ) with that of the general NOS inhibitor N ( G ) - nitro-L-arginine ( L-NA ) in isolated rat basilar arteries ( BAs ) .
	manualset3
156909	5	410191	7	NULL	NULL	NULL	NULL	general NOS inhibitor N ( G ) - nitro-L-arginine ( L-NA )	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The function of the neuronal isoform of nitric oxide synthase ( nNOS ) was studied by comparing the effects of the specific nNOS blocker 7-nitro indazole monosodium salt ( 7-NINA ) with that of the general NOS inhibitor N ( G ) - nitro-L-arginine ( L-NA ) in isolated rat basilar arteries ( BAs ) .
	manualset3
156910	6	410191	7	NULL	NULL	0	NULL	 isolated rat basilar arteries ( BAs )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The function of the neuronal isoform of nitric oxide synthase ( nNOS ) was studied by comparing the effects of the specific nNOS blocker 7-nitro indazole monosodium salt ( 7-NINA ) with that of the general NOS inhibitor N ( G ) - nitro-L-arginine ( L-NA ) in isolated rat basilar arteries ( BAs ) .
	manualset3
157332	7	410191	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The function of the neuronal isoform of nitric oxide synthase ( nNOS ) was studied by comparing the effects of the specific nNOS blocker 7-nitro indazole monosodium salt ( 7-NINA ) with that of the general NOS inhibitor N ( G ) - nitro-L-arginine ( L-NA ) in isolated rat basilar arteries ( BAs ) .
	manualset3
156911	1	410192	7	NULL	NULL	0	NULL	 functional polysaccharide surface	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The functional polysaccharide surface gave similar ELISA results to plates coated passively with the corresponding unmodified lipopolysaccharide antigens .
	manualset3
156912	2	410192	7	NULL	NULL	0	NULL	ELISA results	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The functional polysaccharide surface gave similar ELISA results to plates coated passively with the corresponding unmodified lipopolysaccharide antigens .
	manualset3
156913	4	410192	7	NULL	NULL	NULL	NULL	unmodified lipopolysaccharide antigens	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The functional polysaccharide surface gave similar ELISA results to plates coated passively with the corresponding unmodified lipopolysaccharide antigens .
	manualset3
156914	3	410192	7	NULL	NULL	NULL	NULL	plates	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The functional polysaccharide surface gave similar ELISA results to plates coated passively with the corresponding unmodified lipopolysaccharide antigens .
	manualset3
156915	1	410193	7	NULL	NULL	0	NULL	functional relevance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The functional relevance of leptin-induced nuclear STAT5 activation in hypothalamic cells still has to be determined .
	manualset3
156916	2	410193	7	NULL	NULL	0	NULL	 leptin-induced nuclear STAT5 activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The functional relevance of leptin-induced nuclear STAT5 activation in hypothalamic cells still has to be determined .
	manualset3
156917	3	410193	7	NULL	NULL	0	NULL	hypothalamic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The functional relevance of leptin-induced nuclear STAT5 activation in hypothalamic cells still has to be determined .
	manualset3
156918	1	410194	7	NULL	NULL	0	NULL	survey	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey of the knowledge , attitude and practice of family planning was conducted in Dharan , Nepal .
	manualset3
156919	2	410194	7	NULL	NULL	NULL	NULL	knowledge	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A survey of the knowledge , attitude and practice of family planning was conducted in Dharan , Nepal .
	manualset3
156920	3	410194	7	NULL	NULL	0	NULL	attitude	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey of the knowledge , attitude and practice of family planning was conducted in Dharan , Nepal .
	manualset3
156921	4	410194	7	NULL	NULL	0	NULL	practice of family planning 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey of the knowledge , attitude and practice of family planning was conducted in Dharan , Nepal .
	manualset3
156922	5	410194	7	NULL	NULL	0	NULL	Dharan , Nepal	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey of the knowledge , attitude and practice of family planning was conducted in Dharan , Nepal .
	manualset3
156923	1	410195	7	NULL	NULL	0	NULL	functional significance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The functional significance of the interaction between both proteins was investigated at two different conditions : inactivation of PARP-1 and overexpression of PARP-1 .
	manualset3
156924	2	410195	7	NULL	NULL	0	NULL	interaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The functional significance of the interaction between both proteins was investigated at two different conditions : inactivation of PARP-1 and overexpression of PARP-1 .
	manualset3
156925	3	410195	7	NULL	NULL	0	NULL	proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The functional significance of the interaction between both proteins was investigated at two different conditions : inactivation of PARP-1 and overexpression of PARP-1 .
	manualset3
156926	4	410195	7	NULL	NULL	0	NULL	 different conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The functional significance of the interaction between both proteins was investigated at two different conditions : inactivation of PARP-1 and overexpression of PARP-1 .
	manualset3
156927	5	410195	7	NULL	NULL	0	NULL	inactivation of PARP-1 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The functional significance of the interaction between both proteins was investigated at two different conditions : inactivation of PARP-1 and overexpression of PARP-1 .
	manualset3
156928	6	410195	7	NULL	NULL	0	NULL	overexpression of PARP-1	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The functional significance of the interaction between both proteins was investigated at two different conditions : inactivation of PARP-1 and overexpression of PARP-1 .
	manualset3
156929	1	410196	7	NULL	NULL	0	NULL	 functional state 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The functional state and electrochemical properties of human blood neutrophil leukocytes after their in vitro interaction with Y. pestis cells , strain EV , was analyzed .
	manualset3
156930	2	410196	7	NULL	NULL	0	NULL	electrochemical properties	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The functional state and electrochemical properties of human blood neutrophil leukocytes after their in vitro interaction with Y. pestis cells , strain EV , was analyzed .
	manualset3
156931	3	410196	7	NULL	NULL	0	NULL	human blood neutrophil leukocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The functional state and electrochemical properties of human blood neutrophil leukocytes after their in vitro interaction with Y. pestis cells , strain EV , was analyzed .
	manualset3
156932	4	410196	7	NULL	NULL	NULL	NULL	in vitro interaction 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The functional state and electrochemical properties of human blood neutrophil leukocytes after their in vitro interaction with Y. pestis cells , strain EV , was analyzed .
	manualset3
156934	5	410196	7	NULL	NULL	NULL	NULL	Y. pestis cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The functional state and electrochemical properties of human blood neutrophil leukocytes after their in vitro interaction with Y. pestis cells , strain EV , was analyzed .
	manualset3
156935	6	410196	7	NULL	NULL	NULL	NULL	strain EV	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The functional state and electrochemical properties of human blood neutrophil leukocytes after their in vitro interaction with Y. pestis cells , strain EV , was analyzed .
	manualset3
156936	1	410197	7	NULL	NULL	NULL	NULL	functionality	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The functionality and pathogenicity of these LDGs have not been characterized .
	manualset3
156937	2	410197	7	NULL	NULL	0	NULL	pathogenicity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The functionality and pathogenicity of these LDGs have not been characterized .
	manualset3
156938	3	410197	7	NULL	NULL	0	NULL	LDGs	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The functionality and pathogenicity of these LDGs have not been characterized .
	manualset3
156939	1	410198	7	NULL	NULL	0	NULL	 functionalized terpyridine ligand : 4 ' - ( trans-2-methyl-2-butenoic acid ) - terpyridyl ( L1 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The functionalized terpyridine ligand : 4 ' - ( trans-2-methyl-2-butenoic acid ) - terpyridyl ( L1 ) was synthesized by aryl bromide substitution on terpyridine in a basic reaction condition under palladium carbide catalysis .
	manualset3
156940	2	410198	7	NULL	NULL	NULL	NULL	aryl bromide substitution on terpyridine	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The functionalized terpyridine ligand : 4 ' - ( trans-2-methyl-2-butenoic acid ) - terpyridyl ( L1 ) was synthesized by aryl bromide substitution on terpyridine in a basic reaction condition under palladium carbide catalysis .
	manualset3
156942	3	410198	7	NULL	NULL	NULL	NULL	basic reaction condition	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The functionalized terpyridine ligand : 4 ' - ( trans-2-methyl-2-butenoic acid ) - terpyridyl ( L1 ) was synthesized by aryl bromide substitution on terpyridine in a basic reaction condition under palladium carbide catalysis .
	manualset3
156943	4	410198	7	NULL	NULL	NULL	NULL	palladium carbide catalysis	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The functionalized terpyridine ligand : 4 ' - ( trans-2-methyl-2-butenoic acid ) - terpyridyl ( L1 ) was synthesized by aryl bromide substitution on terpyridine in a basic reaction condition under palladium carbide catalysis .
	manualset3
156944	1	410199	7	NULL	NULL	0	NULL	functions 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The functions , regulation , and mechanisms of action of neuronal RasGRPs are unknown .
	manualset3
156945	2	410199	7	NULL	NULL	0	NULL	regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The functions , regulation , and mechanisms of action of neuronal RasGRPs are unknown .
	manualset3
156946	3	410199	7	NULL	NULL	0	NULL	mechanisms of action	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The functions , regulation , and mechanisms of action of neuronal RasGRPs are unknown .
	manualset3
156947	4	410199	7	NULL	NULL	0	NULL	neuronal RasGRPs	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The functions , regulation , and mechanisms of action of neuronal RasGRPs are unknown .
	manualset3
156948	1	410200	7	NULL	NULL	NULL	NULL	fundamental properties of the theory	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fundamental properties of the theory , i.e. the capability to describe the potential , the field and the concentration/charge density profile within the two classes of materials mentioned above are demonstrated .
	manualset3
156949	2	410200	7	NULL	NULL	0	NULL	capability to describe the potential 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The fundamental properties of the theory , i.e. the capability to describe the potential , the field and the concentration/charge density profile within the two classes of materials mentioned above are demonstrated .
	manualset3
156950	3	410200	7	NULL	NULL	0	NULL	the field	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The fundamental properties of the theory , i.e. the capability to describe the potential , the field and the concentration/charge density profile within the two classes of materials mentioned above are demonstrated .
	manualset3
156951	4	410200	7	NULL	NULL	0	NULL	concentration/charge density profile	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The fundamental properties of the theory , i.e. the capability to describe the potential , the field and the concentration/charge density profile within the two classes of materials mentioned above are demonstrated .
	manualset3
156952	5	410200	7	NULL	NULL	0	NULL	two classes of materials 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The fundamental properties of the theory , i.e. the capability to describe the potential , the field and the concentration/charge density profile within the two classes of materials mentioned above are demonstrated .
	manualset3
156953	1	410201	7	NULL	NULL	0	NULL	fundamental role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The fundamental role of the cellular contacts in the normal function of myelinated fibers has been supported by rodent models and the detection of genetic alterations in patients with peripheral demyelinating neuropathies such as Charcot-Marie-Tooth diseases .
	manualset3
156954	2	410201	7	NULL	NULL	0	NULL	cellular contacts	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The fundamental role of the cellular contacts in the normal function of myelinated fibers has been supported by rodent models and the detection of genetic alterations in patients with peripheral demyelinating neuropathies such as Charcot-Marie-Tooth diseases .
	manualset3
156955	3	410201	7	NULL	NULL	0	NULL	normal function of myelinated fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The fundamental role of the cellular contacts in the normal function of myelinated fibers has been supported by rodent models and the detection of genetic alterations in patients with peripheral demyelinating neuropathies such as Charcot-Marie-Tooth diseases .
	manualset3
156956	4	410201	7	NULL	NULL	0	NULL	rodent models	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The fundamental role of the cellular contacts in the normal function of myelinated fibers has been supported by rodent models and the detection of genetic alterations in patients with peripheral demyelinating neuropathies such as Charcot-Marie-Tooth diseases .
	manualset3
156957	5	410201	7	NULL	NULL	0	NULL	detection of genetic alterations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The fundamental role of the cellular contacts in the normal function of myelinated fibers has been supported by rodent models and the detection of genetic alterations in patients with peripheral demyelinating neuropathies such as Charcot-Marie-Tooth diseases .
	manualset3
156958	6	410201	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The fundamental role of the cellular contacts in the normal function of myelinated fibers has been supported by rodent models and the detection of genetic alterations in patients with peripheral demyelinating neuropathies such as Charcot-Marie-Tooth diseases .
	manualset3
156959	7	410201	7	NULL	NULL	0	NULL	peripheral demyelinating neuropathies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The fundamental role of the cellular contacts in the normal function of myelinated fibers has been supported by rodent models and the detection of genetic alterations in patients with peripheral demyelinating neuropathies such as Charcot-Marie-Tooth diseases .
	manualset3
156960	8	410201	7	NULL	NULL	0	NULL	Charcot-Marie-Tooth diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The fundamental role of the cellular contacts in the normal function of myelinated fibers has been supported by rodent models and the detection of genetic alterations in patients with peripheral demyelinating neuropathies such as Charcot-Marie-Tooth diseases .
	manualset3
156962	1	410202	7	NULL	NULL	0	NULL	fungal enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The fungal enzyme hydrolysed the polysaccharide almost completely to a mixture of the four xyloglucan oligosaccharides : ( formula : see text ) Exhaustive digestion with the nasturtium enzyme gave the same four oligosaccharides plus large amounts of higher oligosaccharides and higher-polymeric material .
	manualset3
156963	2	410202	7	NULL	NULL	0	NULL	polysaccharide 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The fungal enzyme hydrolysed the polysaccharide almost completely to a mixture of the four xyloglucan oligosaccharides : ( formula : see text ) Exhaustive digestion with the nasturtium enzyme gave the same four oligosaccharides plus large amounts of higher oligosaccharides and higher-polymeric material .
	manualset3
156964	3	410202	7	NULL	NULL	0	NULL	mixture of the four xyloglucan oligosaccharides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The fungal enzyme hydrolysed the polysaccharide almost completely to a mixture of the four xyloglucan oligosaccharides : ( formula : see text ) Exhaustive digestion with the nasturtium enzyme gave the same four oligosaccharides plus large amounts of higher oligosaccharides and higher-polymeric material .
	manualset3
156965	4	410202	7	NULL	NULL	0	NULL	formula	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The fungal enzyme hydrolysed the polysaccharide almost completely to a mixture of the four xyloglucan oligosaccharides : ( formula : see text ) Exhaustive digestion with the nasturtium enzyme gave the same four oligosaccharides plus large amounts of higher oligosaccharides and higher-polymeric material .
	manualset3
156966	5	410202	7	NULL	NULL	0	NULL	Exhaustive digestion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The fungal enzyme hydrolysed the polysaccharide almost completely to a mixture of the four xyloglucan oligosaccharides : ( formula : see text ) Exhaustive digestion with the nasturtium enzyme gave the same four oligosaccharides plus large amounts of higher oligosaccharides and higher-polymeric material .
	manualset3
156967	6	410202	7	NULL	NULL	0	NULL	nasturtium enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The fungal enzyme hydrolysed the polysaccharide almost completely to a mixture of the four xyloglucan oligosaccharides : ( formula : see text ) Exhaustive digestion with the nasturtium enzyme gave the same four oligosaccharides plus large amounts of higher oligosaccharides and higher-polymeric material .
	manualset3
156968	7	410202	7	NULL	NULL	0	NULL	four oligosaccharides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The fungal enzyme hydrolysed the polysaccharide almost completely to a mixture of the four xyloglucan oligosaccharides : ( formula : see text ) Exhaustive digestion with the nasturtium enzyme gave the same four oligosaccharides plus large amounts of higher oligosaccharides and higher-polymeric material .
	manualset3
156969	8	410202	7	NULL	NULL	0	NULL	higher oligosaccharides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The fungal enzyme hydrolysed the polysaccharide almost completely to a mixture of the four xyloglucan oligosaccharides : ( formula : see text ) Exhaustive digestion with the nasturtium enzyme gave the same four oligosaccharides plus large amounts of higher oligosaccharides and higher-polymeric material .
	manualset3
156970	9	410202	7	NULL	NULL	0	NULL	higher-polymeric material	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The fungal enzyme hydrolysed the polysaccharide almost completely to a mixture of the four xyloglucan oligosaccharides : ( formula : see text ) Exhaustive digestion with the nasturtium enzyme gave the same four oligosaccharides plus large amounts of higher oligosaccharides and higher-polymeric material .
	manualset3
156971	1	410203	7	NULL	NULL	0	NULL	fungus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The fungus was cultured on yeast extract-sucrose ( YES ) broth in presence of various twofold serial dilutions of 25 % Akacid plus ( 1.5-96 microL/50 mL medium ) and then incubated in shaking condition with 150 rev. / min at 28 degrees C for 96 h. Based on obtained results , Akacid plus was found to significantly inhibit both growth and aflatoxin B1 ( AFB1 ) synthesis in very low concentrations in a dose-dependent manner .
	manualset3
156972	2	410203	7	NULL	NULL	0	NULL	yeast extract-sucrose ( YES ) broth	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The fungus was cultured on yeast extract-sucrose ( YES ) broth in presence of various twofold serial dilutions of 25 % Akacid plus ( 1.5-96 microL/50 mL medium ) and then incubated in shaking condition with 150 rev. / min at 28 degrees C for 96 h. Based on obtained results , Akacid plus was found to significantly inhibit both growth and aflatoxin B1 ( AFB1 ) synthesis in very low concentrations in a dose-dependent manner .
	manualset3
156973	3	410203	7	NULL	NULL	0	NULL	twofold serial dilutions	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The fungus was cultured on yeast extract-sucrose ( YES ) broth in presence of various twofold serial dilutions of 25 % Akacid plus ( 1.5-96 microL/50 mL medium ) and then incubated in shaking condition with 150 rev. / min at 28 degrees C for 96 h. Based on obtained results , Akacid plus was found to significantly inhibit both growth and aflatoxin B1 ( AFB1 ) synthesis in very low concentrations in a dose-dependent manner .
	manualset3
156974	4	410203	7	NULL	NULL	0	NULL	25 % Akacid plus	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The fungus was cultured on yeast extract-sucrose ( YES ) broth in presence of various twofold serial dilutions of 25 % Akacid plus ( 1.5-96 microL/50 mL medium ) and then incubated in shaking condition with 150 rev. / min at 28 degrees C for 96 h. Based on obtained results , Akacid plus was found to significantly inhibit both growth and aflatoxin B1 ( AFB1 ) synthesis in very low concentrations in a dose-dependent manner .
	manualset3
156975	5	410203	7	NULL	NULL	0	NULL	1.5-96 microL/50 mL medium	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The fungus was cultured on yeast extract-sucrose ( YES ) broth in presence of various twofold serial dilutions of 25 % Akacid plus ( 1.5-96 microL/50 mL medium ) and then incubated in shaking condition with 150 rev. / min at 28 degrees C for 96 h. Based on obtained results , Akacid plus was found to significantly inhibit both growth and aflatoxin B1 ( AFB1 ) synthesis in very low concentrations in a dose-dependent manner .
	manualset3
156976	6	410203	7	NULL	NULL	0	NULL	shaking condition	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The fungus was cultured on yeast extract-sucrose ( YES ) broth in presence of various twofold serial dilutions of 25 % Akacid plus ( 1.5-96 microL/50 mL medium ) and then incubated in shaking condition with 150 rev. / min at 28 degrees C for 96 h. Based on obtained results , Akacid plus was found to significantly inhibit both growth and aflatoxin B1 ( AFB1 ) synthesis in very low concentrations in a dose-dependent manner .
	manualset3
156977	7	410203	7	NULL	NULL	0	NULL	150 rev. / min	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The fungus was cultured on yeast extract-sucrose ( YES ) broth in presence of various twofold serial dilutions of 25 % Akacid plus ( 1.5-96 microL/50 mL medium ) and then incubated in shaking condition with 150 rev. / min at 28 degrees C for 96 h. Based on obtained results , Akacid plus was found to significantly inhibit both growth and aflatoxin B1 ( AFB1 ) synthesis in very low concentrations in a dose-dependent manner .
	manualset3
156978	8	410203	7	NULL	NULL	0	NULL	28 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The fungus was cultured on yeast extract-sucrose ( YES ) broth in presence of various twofold serial dilutions of 25 % Akacid plus ( 1.5-96 microL/50 mL medium ) and then incubated in shaking condition with 150 rev. / min at 28 degrees C for 96 h. Based on obtained results , Akacid plus was found to significantly inhibit both growth and aflatoxin B1 ( AFB1 ) synthesis in very low concentrations in a dose-dependent manner .
	manualset3
156979	9	410203	7	NULL	NULL	0	NULL	96 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The fungus was cultured on yeast extract-sucrose ( YES ) broth in presence of various twofold serial dilutions of 25 % Akacid plus ( 1.5-96 microL/50 mL medium ) and then incubated in shaking condition with 150 rev. / min at 28 degrees C for 96 h. Based on obtained results , Akacid plus was found to significantly inhibit both growth and aflatoxin B1 ( AFB1 ) synthesis in very low concentrations in a dose-dependent manner .
	manualset3
156980	10	410203	7	NULL	NULL	0	NULL	Akacid plus	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The fungus was cultured on yeast extract-sucrose ( YES ) broth in presence of various twofold serial dilutions of 25 % Akacid plus ( 1.5-96 microL/50 mL medium ) and then incubated in shaking condition with 150 rev. / min at 28 degrees C for 96 h. Based on obtained results , Akacid plus was found to significantly inhibit both growth and aflatoxin B1 ( AFB1 ) synthesis in very low concentrations in a dose-dependent manner .
	manualset3
156981	11	410203	7	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The fungus was cultured on yeast extract-sucrose ( YES ) broth in presence of various twofold serial dilutions of 25 % Akacid plus ( 1.5-96 microL/50 mL medium ) and then incubated in shaking condition with 150 rev. / min at 28 degrees C for 96 h. Based on obtained results , Akacid plus was found to significantly inhibit both growth and aflatoxin B1 ( AFB1 ) synthesis in very low concentrations in a dose-dependent manner .
	manualset3
156982	12	410203	7	NULL	NULL	NULL	NULL	aflatoxin B1 ( AFB1 ) synthesis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fungus was cultured on yeast extract-sucrose ( YES ) broth in presence of various twofold serial dilutions of 25 % Akacid plus ( 1.5-96 microL/50 mL medium ) and then incubated in shaking condition with 150 rev. / min at 28 degrees C for 96 h. Based on obtained results , Akacid plus was found to significantly inhibit both growth and aflatoxin B1 ( AFB1 ) synthesis in very low concentrations in a dose-dependent manner .
	manualset3
156983	13	410203	7	NULL	NULL	0	NULL	very low concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The fungus was cultured on yeast extract-sucrose ( YES ) broth in presence of various twofold serial dilutions of 25 % Akacid plus ( 1.5-96 microL/50 mL medium ) and then incubated in shaking condition with 150 rev. / min at 28 degrees C for 96 h. Based on obtained results , Akacid plus was found to significantly inhibit both growth and aflatoxin B1 ( AFB1 ) synthesis in very low concentrations in a dose-dependent manner .
	manualset3
156984	14	410203	7	NULL	NULL	0	NULL	dose-dependent manner	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The fungus was cultured on yeast extract-sucrose ( YES ) broth in presence of various twofold serial dilutions of 25 % Akacid plus ( 1.5-96 microL/50 mL medium ) and then incubated in shaking condition with 150 rev. / min at 28 degrees C for 96 h. Based on obtained results , Akacid plus was found to significantly inhibit both growth and aflatoxin B1 ( AFB1 ) synthesis in very low concentrations in a dose-dependent manner .
	manualset3
156985	1	410204	7	NULL	NULL	0	NULL	survey	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey was administered to a sample of the US population to explore public preferences for types of benefits often associated with biodiversity : utilitarian ( commodity and recreation ) , ecological ( certain and uncertain ) , aesthetic , symbolic , and humanistic .
	manualset3
156986	2	410204	7	NULL	NULL	NULL	NULL	sample of the US population	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A survey was administered to a sample of the US population to explore public preferences for types of benefits often associated with biodiversity : utilitarian ( commodity and recreation ) , ecological ( certain and uncertain ) , aesthetic , symbolic , and humanistic .
	manualset3
156988	3	410204	7	NULL	NULL	NULL	NULL	biodiversity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A survey was administered to a sample of the US population to explore public preferences for types of benefits often associated with biodiversity : utilitarian ( commodity and recreation ) , ecological ( certain and uncertain ) , aesthetic , symbolic , and humanistic .
	manualset3
157333	4	410204	7	NULL	NULL	0	NULL	public preferences	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey was administered to a sample of the US population to explore public preferences for types of benefits often associated with biodiversity : utilitarian ( commodity and recreation ) , ecological ( certain and uncertain ) , aesthetic , symbolic , and humanistic .
	manualset3
156995	1	410205	7	NULL	NULL	0	NULL	furation of estrus	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The furation of estrus and the interval from ovulation to end of estrus were similar among the three treatment groups .
	manualset3
156996	2	410205	7	NULL	NULL	0	NULL	interval from ovulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The furation of estrus and the interval from ovulation to end of estrus were similar among the three treatment groups .
	manualset3
156997	3	410205	7	NULL	NULL	0	NULL	end of estrus 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The furation of estrus and the interval from ovulation to end of estrus were similar among the three treatment groups .
	manualset3
156998	4	410205	7	NULL	NULL	0	NULL	three treatment groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The furation of estrus and the interval from ovulation to end of estrus were similar among the three treatment groups .
	manualset3
156999	1	410206	7	NULL	NULL	0	NULL	further elucidation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The further elucidation of the rhesus macaque MHC and the search for other relevant genes will remain an important task for future research and will stimulate all immunologically-related investigations in macaques .
	manualset3
157000	2	410206	7	NULL	NULL	0	NULL	rhesus macaque MHC	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The further elucidation of the rhesus macaque MHC and the search for other relevant genes will remain an important task for future research and will stimulate all immunologically-related investigations in macaques .
	manualset3
157001	3	410206	7	NULL	NULL	0	NULL	relevant genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The further elucidation of the rhesus macaque MHC and the search for other relevant genes will remain an important task for future research and will stimulate all immunologically-related investigations in macaques .
	manualset3
157002	4	410206	7	NULL	NULL	0	NULL	 important task	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The further elucidation of the rhesus macaque MHC and the search for other relevant genes will remain an important task for future research and will stimulate all immunologically-related investigations in macaques .
	manualset3
157003	5	410206	7	NULL	NULL	0	NULL	future research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The further elucidation of the rhesus macaque MHC and the search for other relevant genes will remain an important task for future research and will stimulate all immunologically-related investigations in macaques .
	manualset3
157005	7	410206	7	NULL	NULL	0	NULL	 immunologically-related investigations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The further elucidation of the rhesus macaque MHC and the search for other relevant genes will remain an important task for future research and will stimulate all immunologically-related investigations in macaques .
	manualset3
157006	8	410206	7	NULL	NULL	0	NULL	macaques	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The further elucidation of the rhesus macaque MHC and the search for other relevant genes will remain an important task for future research and will stimulate all immunologically-related investigations in macaques .
	manualset3
157334	9	410206	7	NULL	NULL	0	NULL	search	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The further elucidation of the rhesus macaque MHC and the search for other relevant genes will remain an important task for future research and will stimulate all immunologically-related investigations in macaques .
	manualset3
157007	1	410207	7	NULL	NULL	0	NULL	fusion gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The fusion gene contains a presumptive sequence for mitochondrial import from the mitochondrial tyrosyl-tRNA synthetase gene fused to the E. coli coding region .
	manualset3
157008	2	410207	7	NULL	NULL	0	NULL	presumptive sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The fusion gene contains a presumptive sequence for mitochondrial import from the mitochondrial tyrosyl-tRNA synthetase gene fused to the E. coli coding region .
	manualset3
157009	3	410207	7	NULL	NULL	0	NULL	mitochondrial import 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The fusion gene contains a presumptive sequence for mitochondrial import from the mitochondrial tyrosyl-tRNA synthetase gene fused to the E. coli coding region .
	manualset3
157010	4	410207	7	NULL	NULL	0	NULL	mitochondrial tyrosyl-tRNA synthetase gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The fusion gene contains a presumptive sequence for mitochondrial import from the mitochondrial tyrosyl-tRNA synthetase gene fused to the E. coli coding region .
	manualset3
157011	5	410207	7	NULL	NULL	0	NULL	E. coli coding region	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The fusion gene contains a presumptive sequence for mitochondrial import from the mitochondrial tyrosyl-tRNA synthetase gene fused to the E. coli coding region .
	manualset3
157012	1	410208	7	NULL	NULL	NULL	NULL	fusion of cloned mouse myoblasts	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fusion of cloned mouse myoblasts was markedly inhibited , in a dose-dependent manner , when cells were cultured in medium supplemented with either phenidone ( 1-phenyl-3-pyrazolidione ) or BW755c ( 3-amino-1 - ( 3-tri-fluoromethylphenyl ) -2 - pyrazoline ) , drugs which have been reported to inhibit lipoxygenase and cyclo-oxygenase activities .
	manualset3
157013	2	410208	7	NULL	NULL	0	NULL	dose-dependent manner	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The fusion of cloned mouse myoblasts was markedly inhibited , in a dose-dependent manner , when cells were cultured in medium supplemented with either phenidone ( 1-phenyl-3-pyrazolidione ) or BW755c ( 3-amino-1 - ( 3-tri-fluoromethylphenyl ) -2 - pyrazoline ) , drugs which have been reported to inhibit lipoxygenase and cyclo-oxygenase activities .
	manualset3
157014	3	410208	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The fusion of cloned mouse myoblasts was markedly inhibited , in a dose-dependent manner , when cells were cultured in medium supplemented with either phenidone ( 1-phenyl-3-pyrazolidione ) or BW755c ( 3-amino-1 - ( 3-tri-fluoromethylphenyl ) -2 - pyrazoline ) , drugs which have been reported to inhibit lipoxygenase and cyclo-oxygenase activities .
	manualset3
157015	4	410208	7	NULL	NULL	0	NULL	medium	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The fusion of cloned mouse myoblasts was markedly inhibited , in a dose-dependent manner , when cells were cultured in medium supplemented with either phenidone ( 1-phenyl-3-pyrazolidione ) or BW755c ( 3-amino-1 - ( 3-tri-fluoromethylphenyl ) -2 - pyrazoline ) , drugs which have been reported to inhibit lipoxygenase and cyclo-oxygenase activities .
	manualset3
157016	5	410208	7	NULL	NULL	NULL	NULL	phenidone ( 1-phenyl-3-pyrazolidione )	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fusion of cloned mouse myoblasts was markedly inhibited , in a dose-dependent manner , when cells were cultured in medium supplemented with either phenidone ( 1-phenyl-3-pyrazolidione ) or BW755c ( 3-amino-1 - ( 3-tri-fluoromethylphenyl ) -2 - pyrazoline ) , drugs which have been reported to inhibit lipoxygenase and cyclo-oxygenase activities .
	manualset3
157017	6	410208	7	NULL	NULL	0	NULL	BW755c ( 3-amino-1 - ( 3-tri-fluoromethylphenyl ) -2 - pyrazoline ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The fusion of cloned mouse myoblasts was markedly inhibited , in a dose-dependent manner , when cells were cultured in medium supplemented with either phenidone ( 1-phenyl-3-pyrazolidione ) or BW755c ( 3-amino-1 - ( 3-tri-fluoromethylphenyl ) -2 - pyrazoline ) , drugs which have been reported to inhibit lipoxygenase and cyclo-oxygenase activities .
	manualset3
157018	7	410208	7	NULL	NULL	0	NULL	drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The fusion of cloned mouse myoblasts was markedly inhibited , in a dose-dependent manner , when cells were cultured in medium supplemented with either phenidone ( 1-phenyl-3-pyrazolidione ) or BW755c ( 3-amino-1 - ( 3-tri-fluoromethylphenyl ) -2 - pyrazoline ) , drugs which have been reported to inhibit lipoxygenase and cyclo-oxygenase activities .
	manualset3
157019	8	410208	7	NULL	NULL	0	NULL	lipoxygenase activities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The fusion of cloned mouse myoblasts was markedly inhibited , in a dose-dependent manner , when cells were cultured in medium supplemented with either phenidone ( 1-phenyl-3-pyrazolidione ) or BW755c ( 3-amino-1 - ( 3-tri-fluoromethylphenyl ) -2 - pyrazoline ) , drugs which have been reported to inhibit lipoxygenase and cyclo-oxygenase activities .
	manualset3
157020	9	410208	7	NULL	NULL	0	NULL	cyclo-oxygenase activities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The fusion of cloned mouse myoblasts was markedly inhibited , in a dose-dependent manner , when cells were cultured in medium supplemented with either phenidone ( 1-phenyl-3-pyrazolidione ) or BW755c ( 3-amino-1 - ( 3-tri-fluoromethylphenyl ) -2 - pyrazoline ) , drugs which have been reported to inhibit lipoxygenase and cyclo-oxygenase activities .
	manualset3
157021	1	410209	7	NULL	NULL	0	NULL	fusion protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The fusion protein showed specific binding to IL-8 receptors , induced IL-8 mediated chemotactic activity , and the release of MPO activity .
	manualset3
157022	2	410209	7	NULL	NULL	0	NULL	specific binding	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The fusion protein showed specific binding to IL-8 receptors , induced IL-8 mediated chemotactic activity , and the release of MPO activity .
	manualset3
157023	3	410209	7	NULL	NULL	0	NULL	IL-8 receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The fusion protein showed specific binding to IL-8 receptors , induced IL-8 mediated chemotactic activity , and the release of MPO activity .
	manualset3
157024	4	410209	7	NULL	NULL	0	NULL	 IL-8 mediated chemotactic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The fusion protein showed specific binding to IL-8 receptors , induced IL-8 mediated chemotactic activity , and the release of MPO activity .
	manualset3
157025	5	410209	7	NULL	NULL	0	NULL	release of MPO activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The fusion protein showed specific binding to IL-8 receptors , induced IL-8 mediated chemotactic activity , and the release of MPO activity .
	manualset3
157026	1	410210	7	NULL	NULL	0	NULL	 future	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The future of primary care paediatrics and child health .
	manualset3
157027	2	410210	7	NULL	NULL	0	NULL	primary care paediatrics	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The future of primary care paediatrics and child health .
	manualset3
157028	3	410210	7	NULL	NULL	0	NULL	child health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The future of primary care paediatrics and child health .
	manualset3
157029	1	410211	7	NULL	NULL	0	NULL	Clinical and angiographic predicting factors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical and angiographic predicting factors leading to unfavorable myocardial reperfusion in patients with acute ST-elevation myocardial infarction after primary percutaneous coronary intervention ) .
	manualset3
157030	2	410211	7	NULL	NULL	0	NULL	unfavorable myocardial reperfusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical and angiographic predicting factors leading to unfavorable myocardial reperfusion in patients with acute ST-elevation myocardial infarction after primary percutaneous coronary intervention ) .
	manualset3
157031	3	410211	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical and angiographic predicting factors leading to unfavorable myocardial reperfusion in patients with acute ST-elevation myocardial infarction after primary percutaneous coronary intervention ) .
	manualset3
157032	4	410211	7	NULL	NULL	0	NULL	acute ST-elevation myocardial infarction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical and angiographic predicting factors leading to unfavorable myocardial reperfusion in patients with acute ST-elevation myocardial infarction after primary percutaneous coronary intervention ) .
	manualset3
157033	5	410211	7	NULL	NULL	0	NULL	primary percutaneous coronary intervention	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical and angiographic predicting factors leading to unfavorable myocardial reperfusion in patients with acute ST-elevation myocardial infarction after primary percutaneous coronary intervention ) .
	manualset3
157034	1	410212	7	NULL	NULL	0	NULL	survey	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey was conducted in 1998-2001 among 715 Polish seafarers examined at the Institute of Maritime and Tropical Medicine in Gdynia .
	manualset3
157035	2	410212	7	NULL	NULL	0	NULL	1998-2001	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey was conducted in 1998-2001 among 715 Polish seafarers examined at the Institute of Maritime and Tropical Medicine in Gdynia .
	manualset3
157036	3	410212	7	NULL	NULL	0	NULL	715 Polish seafarers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey was conducted in 1998-2001 among 715 Polish seafarers examined at the Institute of Maritime and Tropical Medicine in Gdynia .
	manualset3
157037	4	410212	7	NULL	NULL	0	NULL	Institute of Maritime and Tropical Medicine	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey was conducted in 1998-2001 among 715 Polish seafarers examined at the Institute of Maritime and Tropical Medicine in Gdynia .
	manualset3
157038	5	410212	7	NULL	NULL	0	NULL	Gdynia 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey was conducted in 1998-2001 among 715 Polish seafarers examined at the Institute of Maritime and Tropical Medicine in Gdynia .
	manualset3
157039	1	410213	7	NULL	NULL	0	NULL	gamma-aminobutyric acid-alpha-ketoglutaric acid transaminase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The gamma-aminobutyric acid-alpha-ketoglutaric acid transaminase of beef brain .
	manualset3
157040	2	410213	7	NULL	NULL	0	NULL	beef brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The gamma-aminobutyric acid-alpha-ketoglutaric acid transaminase of beef brain .
	manualset3
157041	1	410214	7	NULL	NULL	0	NULL	gamma3 subunit	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The gamma3 subunit is involved in the regulation of AMPK activity in skeletal muscle and strongly influences glycogen metabolism .
	manualset3
157042	2	410214	7	NULL	NULL	NULL	NULL	 regulation of AMPK activity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The gamma3 subunit is involved in the regulation of AMPK activity in skeletal muscle and strongly influences glycogen metabolism .
	manualset3
157044	4	410214	7	NULL	NULL	0	NULL	skeletal muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The gamma3 subunit is involved in the regulation of AMPK activity in skeletal muscle and strongly influences glycogen metabolism .
	manualset3
157045	5	410214	7	NULL	NULL	0	NULL	glycogen metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The gamma3 subunit is involved in the regulation of AMPK activity in skeletal muscle and strongly influences glycogen metabolism .
	manualset3
157046	1	410215	7	NULL	NULL	0	NULL	gastric lumen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The gastric lumen of the fetal rat at the 20th day of gestation contained a statistically significant amount of basal pepsin , which increased log linearly over the first 30 days of life .
	manualset3
157047	2	410215	7	NULL	NULL	0	NULL	fetal rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The gastric lumen of the fetal rat at the 20th day of gestation contained a statistically significant amount of basal pepsin , which increased log linearly over the first 30 days of life .
	manualset3
157048	3	410215	7	NULL	NULL	NULL	NULL	20th day of gestation	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The gastric lumen of the fetal rat at the 20th day of gestation contained a statistically significant amount of basal pepsin , which increased log linearly over the first 30 days of life .
	manualset3
157049	4	410215	7	NULL	NULL	0	NULL	basal pepsin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The gastric lumen of the fetal rat at the 20th day of gestation contained a statistically significant amount of basal pepsin , which increased log linearly over the first 30 days of life .
	manualset3
157051	6	410215	7	NULL	NULL	0	NULL	first 30 days of life	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The gastric lumen of the fetal rat at the 20th day of gestation contained a statistically significant amount of basal pepsin , which increased log linearly over the first 30 days of life .
	manualset3
157052	1	410216	7	NULL	NULL	0	NULL	gastric mucosa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The gastric mucosa was exposed , chambered , and continuously superfused with buffers under in vivo microscopy .
	manualset3
157055	2	410216	7	NULL	NULL	NULL	NULL	 buffers	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The gastric mucosa was exposed , chambered , and continuously superfused with buffers under in vivo microscopy .
	manualset3
157056	3	410216	7	NULL	NULL	NULL	NULL	in vivo microscopy	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The gastric mucosa was exposed , chambered , and continuously superfused with buffers under in vivo microscopy .
	manualset3
157057	1	410217	7	NULL	NULL	0	NULL	gastrocnemius muscle contractility	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The gastrocnemius muscle contractility was also examined prior to euthanasia at 91 days postsurgery in all groups using electromyography .
	manualset3
157058	2	410217	7	NULL	NULL	0	NULL	euthanasia	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The gastrocnemius muscle contractility was also examined prior to euthanasia at 91 days postsurgery in all groups using electromyography .
	manualset3
157059	3	410217	7	NULL	NULL	NULL	NULL	91 days postsurgery	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The gastrocnemius muscle contractility was also examined prior to euthanasia at 91 days postsurgery in all groups using electromyography .
	manualset3
157060	4	410217	7	NULL	NULL	0	NULL	groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The gastrocnemius muscle contractility was also examined prior to euthanasia at 91 days postsurgery in all groups using electromyography .
	manualset3
157061	5	410217	7	NULL	NULL	0	NULL	electromyography	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The gastrocnemius muscle contractility was also examined prior to euthanasia at 91 days postsurgery in all groups using electromyography .
	manualset3
157062	1	410218	7	NULL	NULL	0	NULL	gel	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The gel was then dipped in a 50 mM Tris-HCl buffer ( pH 7.9 ) containing 4.0 mM oxidized glutathione ( GSSG ) , 1.5 mM NADPH , and 2 mM 5 , 5 ' - dithiobis ( 2-nitrobenzoic acid ) ( DTNB ) for 20 min .
	manualset3
157063	2	410218	7	NULL	NULL	0	NULL	50 mM Tris-HCl buffer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The gel was then dipped in a 50 mM Tris-HCl buffer ( pH 7.9 ) containing 4.0 mM oxidized glutathione ( GSSG ) , 1.5 mM NADPH , and 2 mM 5 , 5 ' - dithiobis ( 2-nitrobenzoic acid ) ( DTNB ) for 20 min .
	manualset3
157064	3	410218	7	NULL	NULL	0	NULL	 pH 7.9	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The gel was then dipped in a 50 mM Tris-HCl buffer ( pH 7.9 ) containing 4.0 mM oxidized glutathione ( GSSG ) , 1.5 mM NADPH , and 2 mM 5 , 5 ' - dithiobis ( 2-nitrobenzoic acid ) ( DTNB ) for 20 min .
	manualset3
157065	4	410218	7	NULL	NULL	0	NULL	4.0 mM oxidized glutathione ( GSSG )	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The gel was then dipped in a 50 mM Tris-HCl buffer ( pH 7.9 ) containing 4.0 mM oxidized glutathione ( GSSG ) , 1.5 mM NADPH , and 2 mM 5 , 5 ' - dithiobis ( 2-nitrobenzoic acid ) ( DTNB ) for 20 min .
	manualset3
157066	5	410218	7	NULL	NULL	0	NULL	1.5 mM NADPH	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The gel was then dipped in a 50 mM Tris-HCl buffer ( pH 7.9 ) containing 4.0 mM oxidized glutathione ( GSSG ) , 1.5 mM NADPH , and 2 mM 5 , 5 ' - dithiobis ( 2-nitrobenzoic acid ) ( DTNB ) for 20 min .
	manualset3
157067	6	410218	7	NULL	NULL	0	NULL	2 mM 5 , 5 ' - dithiobis ( 2-nitrobenzoic acid ) ( DTNB )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The gel was then dipped in a 50 mM Tris-HCl buffer ( pH 7.9 ) containing 4.0 mM oxidized glutathione ( GSSG ) , 1.5 mM NADPH , and 2 mM 5 , 5 ' - dithiobis ( 2-nitrobenzoic acid ) ( DTNB ) for 20 min .
	manualset3
157068	7	410218	7	NULL	NULL	0	NULL	20 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The gel was then dipped in a 50 mM Tris-HCl buffer ( pH 7.9 ) containing 4.0 mM oxidized glutathione ( GSSG ) , 1.5 mM NADPH , and 2 mM 5 , 5 ' - dithiobis ( 2-nitrobenzoic acid ) ( DTNB ) for 20 min .
	manualset3
157069	1	410219	7	NULL	NULL	0	NULL	gene-rich region	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene-rich region is flanked at the proximal and distal ends by retrotransposon blocks .
	manualset3
157070	2	410219	7	NULL	NULL	NULL	NULL	proximal ends	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The gene-rich region is flanked at the proximal and distal ends by retrotransposon blocks .
	manualset3
157071	3	410219	7	NULL	NULL	NULL	NULL	distal ends	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The gene-rich region is flanked at the proximal and distal ends by retrotransposon blocks .
	manualset3
157072	4	410219	7	NULL	NULL	0	NULL	retrotransposon blocks	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene-rich region is flanked at the proximal and distal ends by retrotransposon blocks .
	manualset3
157073	1	410220	7	NULL	NULL	0	NULL	gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene coding for insulin-like growth factor-binding protein 3 ( IGFBP3 ) is important for regulation of growth , development and metabolism in mammals .
	manualset3
157074	2	410220	7	NULL	NULL	0	NULL	 insulin-like growth factor-binding protein 3 ( IGFBP3 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene coding for insulin-like growth factor-binding protein 3 ( IGFBP3 ) is important for regulation of growth , development and metabolism in mammals .
	manualset3
157075	3	410220	7	NULL	NULL	0	NULL	regulation of growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene coding for insulin-like growth factor-binding protein 3 ( IGFBP3 ) is important for regulation of growth , development and metabolism in mammals .
	manualset3
157076	4	410220	7	NULL	NULL	0	NULL	development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene coding for insulin-like growth factor-binding protein 3 ( IGFBP3 ) is important for regulation of growth , development and metabolism in mammals .
	manualset3
157077	5	410220	7	NULL	NULL	0	NULL	metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene coding for insulin-like growth factor-binding protein 3 ( IGFBP3 ) is important for regulation of growth , development and metabolism in mammals .
	manualset3
157078	6	410220	7	NULL	NULL	0	NULL	mammals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene coding for insulin-like growth factor-binding protein 3 ( IGFBP3 ) is important for regulation of growth , development and metabolism in mammals .
	manualset3
157079	1	410221	7	NULL	NULL	0	NULL	survey	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey was conducted on a purposive sample of 34 ex-student nurses who had recently completed their basic nursing course .
	manualset3
157080	2	410221	7	NULL	NULL	NULL	NULL	purposive sample 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A survey was conducted on a purposive sample of 34 ex-student nurses who had recently completed their basic nursing course .
	manualset3
157081	3	410221	7	NULL	NULL	0	NULL	34 ex-student nurses	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey was conducted on a purposive sample of 34 ex-student nurses who had recently completed their basic nursing course .
	manualset3
157082	4	410221	7	NULL	NULL	0	NULL	basic nursing course	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey was conducted on a purposive sample of 34 ex-student nurses who had recently completed their basic nursing course .
	manualset3
157083	1	410222	7	NULL	NULL	0	NULL	gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene donated to germ plasm line KS96WGRC36 from TA 870 of T. timopheevii subsp .
	manualset3
157084	2	410222	7	NULL	NULL	NULL	NULL	germ plasm line KS96WGRC36	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The gene donated to germ plasm line KS96WGRC36 from TA 870 of T. timopheevii subsp .
	manualset3
157085	3	410222	7	NULL	NULL	0	NULL	TA 870 of T. timopheevii subsp	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene donated to germ plasm line KS96WGRC36 from TA 870 of T. timopheevii subsp .
	manualset3
157086	1	410223	7	NULL	NULL	0	NULL	gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene encoding the Pyrococcus furiosus hyperthermophilic amylopullulanase ( APU ) was cloned , sequenced , and expressed in Escherichia coli .
	manualset3
157087	2	410223	7	NULL	NULL	0	NULL	Pyrococcus furiosus hyperthermophilic amylopullulanase ( APU )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene encoding the Pyrococcus furiosus hyperthermophilic amylopullulanase ( APU ) was cloned , sequenced , and expressed in Escherichia coli .
	manualset3
157090	3	410223	7	NULL	NULL	NULL	NULL	Escherichia coli 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The gene encoding the Pyrococcus furiosus hyperthermophilic amylopullulanase ( APU ) was cloned , sequenced , and expressed in Escherichia coli .
	manualset3
157092	2	410224	7	NULL	NULL	NULL	NULL	gene encoding the neopullulanase ( susA )	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The gene encoding the neopullulanase ( susA ) was located upstream of the gene encoding the alpha-glucosidase ( susB ) .
	manualset3
157093	3	410224	7	NULL	NULL	NULL	NULL	upstream	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The gene encoding the neopullulanase ( susA ) was located upstream of the gene encoding the alpha-glucosidase ( susB ) .
	manualset3
157094	4	410224	7	NULL	NULL	NULL	NULL	gene encoding the alpha-glucosidase ( susB )	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The gene encoding the neopullulanase ( susA ) was located upstream of the gene encoding the alpha-glucosidase ( susB ) .
	manualset3
157097	1	410225	7	NULL	NULL	NULL	NULL	gene for M. hemolytica outer membrane protein ( OMP ) PlpE	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The gene for M. hemolytica outer membrane protein ( OMP ) PlpE was cloned into the expression vector pRSETA .
	manualset3
157098	2	410225	7	NULL	NULL	NULL	NULL	expression vector pRSETA	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The gene for M. hemolytica outer membrane protein ( OMP ) PlpE was cloned into the expression vector pRSETA .
	manualset3
157100	1	410226	7	NULL	NULL	NULL	NULL	gene for isocitrate lyase	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The gene for isocitrate lyase from Escherichia coli has recently been cloned and sequenced .
	manualset3
157101	3	410226	7	NULL	NULL	0	NULL	Escherichia coli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene for isocitrate lyase from Escherichia coli has recently been cloned and sequenced .
	manualset3
157104	1	410227	7	NULL	NULL	0	NULL	gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene was located on chromosome 18p11 .2 , adjacent to the G protein Golf alpha gene ( GNAL ) , in tail-to-tail orientation , partially overlapping with the 3 ' UTR of the latter gene .
	manualset3
157105	2	410227	7	NULL	NULL	0	NULL	chromosome 18p11 .2	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene was located on chromosome 18p11 .2 , adjacent to the G protein Golf alpha gene ( GNAL ) , in tail-to-tail orientation , partially overlapping with the 3 ' UTR of the latter gene .
	manualset3
157106	3	410227	7	NULL	NULL	0	NULL	G protein Golf alpha gene ( GNAL )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene was located on chromosome 18p11 .2 , adjacent to the G protein Golf alpha gene ( GNAL ) , in tail-to-tail orientation , partially overlapping with the 3 ' UTR of the latter gene .
	manualset3
157107	4	410227	7	NULL	NULL	0	NULL	 tail-to-tail orientation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene was located on chromosome 18p11 .2 , adjacent to the G protein Golf alpha gene ( GNAL ) , in tail-to-tail orientation , partially overlapping with the 3 ' UTR of the latter gene .
	manualset3
157108	5	410227	7	NULL	NULL	0	NULL	3 ' UTR of the latter gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene was located on chromosome 18p11 .2 , adjacent to the G protein Golf alpha gene ( GNAL ) , in tail-to-tail orientation , partially overlapping with the 3 ' UTR of the latter gene .
	manualset3
157109	1	410228	7	NULL	NULL	0	NULL	 general patterns	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The general patterns of the follicular epithelium changings are similar in the both groups of birds .
	manualset3
157110	2	410228	7	NULL	NULL	0	NULL	follicular epithelium changings	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The general patterns of the follicular epithelium changings are similar in the both groups of birds .
	manualset3
157111	3	410228	7	NULL	NULL	0	NULL	groups of birds	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The general patterns of the follicular epithelium changings are similar in the both groups of birds .
	manualset3
157112	1	410229	7	NULL	NULL	0	NULL	survey	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey was done among 176 Spanish general hospitals over 100 beds .
	manualset3
157113	2	410229	7	NULL	NULL	0	NULL	176 Spanish general hospitals	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey was done among 176 Spanish general hospitals over 100 beds .
	manualset3
157114	3	410229	7	NULL	NULL	0	NULL	100 beds	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey was done among 176 Spanish general hospitals over 100 beds .
	manualset3
157115	1	410230	7	NULL	NULL	NULL	NULL	generic name	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The generic name of the given trade-names were known on average by 83 % of the physicians who had recently prescribed them , but knowledge of the combination drugs was poor .
	manualset3
157116	2	410230	7	NULL	NULL	NULL	NULL	trade-names	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The generic name of the given trade-names were known on average by 83 % of the physicians who had recently prescribed them , but knowledge of the combination drugs was poor .
	manualset3
157117	3	410230	7	NULL	NULL	0	NULL	83 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The generic name of the given trade-names were known on average by 83 % of the physicians who had recently prescribed them , but knowledge of the combination drugs was poor .
	manualset3
157118	4	410230	7	NULL	NULL	0	NULL	physicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The generic name of the given trade-names were known on average by 83 % of the physicians who had recently prescribed them , but knowledge of the combination drugs was poor .
	manualset3
157119	5	410230	7	NULL	NULL	0	NULL	combination drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The generic name of the given trade-names were known on average by 83 % of the physicians who had recently prescribed them , but knowledge of the combination drugs was poor .
	manualset3
157197	6	410230	7	NULL	NULL	0	NULL	poor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The generic name of the given trade-names were known on average by 83 % of the physicians who had recently prescribed them , but knowledge of the combination drugs was poor .
	manualset3
157335	7	410230	7	NULL	NULL	0	NULL	knowledge	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The generic name of the given trade-names were known on average by 83 % of the physicians who had recently prescribed them , but knowledge of the combination drugs was poor .
	manualset3
157120	1	410231	7	NULL	NULL	0	NULL	gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The genes are thus located at 16.8 min in the E. coli linkage map , together with the citrate synthase ( gltA ) and succinate dehydrogenase ( sdh ) genes , in a cluster of nine citric acid cycle genes : gltA-sdhCDAB-sucABCD .
	manualset3
157121	2	410231	7	NULL	NULL	NULL	NULL	16.8 min	Unit												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The genes are thus located at 16.8 min in the E. coli linkage map , together with the citrate synthase ( gltA ) and succinate dehydrogenase ( sdh ) genes , in a cluster of nine citric acid cycle genes : gltA-sdhCDAB-sucABCD .
	manualset3
157122	3	410231	7	NULL	NULL	0	NULL	E. coli linkage map	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The genes are thus located at 16.8 min in the E. coli linkage map , together with the citrate synthase ( gltA ) and succinate dehydrogenase ( sdh ) genes , in a cluster of nine citric acid cycle genes : gltA-sdhCDAB-sucABCD .
	manualset3
157123	4	410231	7	NULL	NULL	0	NULL	citrate synthase ( gltA ) genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The genes are thus located at 16.8 min in the E. coli linkage map , together with the citrate synthase ( gltA ) and succinate dehydrogenase ( sdh ) genes , in a cluster of nine citric acid cycle genes : gltA-sdhCDAB-sucABCD .
	manualset3
157124	5	410231	7	NULL	NULL	0	NULL	succinate dehydrogenase ( sdh ) genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The genes are thus located at 16.8 min in the E. coli linkage map , together with the citrate synthase ( gltA ) and succinate dehydrogenase ( sdh ) genes , in a cluster of nine citric acid cycle genes : gltA-sdhCDAB-sucABCD .
	manualset3
157125	6	410231	7	NULL	NULL	NULL	NULL	cluster of nine citric acid cycle genes 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The genes are thus located at 16.8 min in the E. coli linkage map , together with the citrate synthase ( gltA ) and succinate dehydrogenase ( sdh ) genes , in a cluster of nine citric acid cycle genes : gltA-sdhCDAB-sucABCD .
	manualset3
157126	7	410231	7	NULL	NULL	NULL	NULL	gltA-sdhCDAB-sucABCD	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The genes are thus located at 16.8 min in the E. coli linkage map , together with the citrate synthase ( gltA ) and succinate dehydrogenase ( sdh ) genes , in a cluster of nine citric acid cycle genes : gltA-sdhCDAB-sucABCD .
	manualset3
157127	1	410232	7	NULL	NULL	0	NULL	genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The genes coding the different chains of type IV collagen have been cloned and several mutations have been characterized .
	manualset3
157128	2	410232	7	NULL	NULL	0	NULL	different chains of type IV collagen 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The genes coding the different chains of type IV collagen have been cloned and several mutations have been characterized .
	manualset3
157130	3	410232	7	NULL	NULL	NULL	NULL	several mutations	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The genes coding the different chains of type IV collagen have been cloned and several mutations have been characterized .
	manualset3
157131	1	410233	7	NULL	NULL	0	NULL	genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The genes encoding the subunit proteins of SfaII were identified and sequenced .
	manualset3
157132	2	410233	7	NULL	NULL	0	NULL	subunit proteins	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The genes encoding the subunit proteins of SfaII were identified and sequenced .
	manualset3
157133	3	410233	7	NULL	NULL	0	NULL	 SfaII	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The genes encoding the subunit proteins of SfaII were identified and sequenced .
	manualset3
157136	1	410234	7	NULL	NULL	0	NULL	genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The genes identified included several angiogenic signalling pathways , such as VEGF , FGF and HGF .
	manualset3
157137	2	410234	7	NULL	NULL	NULL	NULL	several angiogenic signalling pathways	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The genes identified included several angiogenic signalling pathways , such as VEGF , FGF and HGF .
	manualset3
157138	3	410234	7	NULL	NULL	0	NULL	VEGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The genes identified included several angiogenic signalling pathways , such as VEGF , FGF and HGF .
	manualset3
157139	4	410234	7	NULL	NULL	0	NULL	FGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The genes identified included several angiogenic signalling pathways , such as VEGF , FGF and HGF .
	manualset3
157140	5	410234	7	NULL	NULL	0	NULL	HGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The genes identified included several angiogenic signalling pathways , such as VEGF , FGF and HGF .
	manualset3
157141	1	410235	7	NULL	NULL	0	NULL	genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The genes responsible for ADPKD , PKD1 , and PKD2 have been identified , and the pathological processes of the disease are becoming clearer .
	manualset3
157142	2	410235	7	NULL	NULL	0	NULL	ADPKD	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The genes responsible for ADPKD , PKD1 , and PKD2 have been identified , and the pathological processes of the disease are becoming clearer .
	manualset3
157143	3	410235	7	NULL	NULL	0	NULL	PKD1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The genes responsible for ADPKD , PKD1 , and PKD2 have been identified , and the pathological processes of the disease are becoming clearer .
	manualset3
157144	4	410235	7	NULL	NULL	0	NULL	PKD2	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The genes responsible for ADPKD , PKD1 , and PKD2 have been identified , and the pathological processes of the disease are becoming clearer .
	manualset3
157145	5	410235	7	NULL	NULL	0	NULL	pathological processes of the disease	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The genes responsible for ADPKD , PKD1 , and PKD2 have been identified , and the pathological processes of the disease are becoming clearer .
	manualset3
157146	1	410236	7	NULL	NULL	NULL	NULL	genes that encode the alpha and beta subunits of protocatechuate 3 , 4-dioxygenase ( 3 , 4-PCD ( EC 1.13.11.3 ) )	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The genes that encode the alpha and beta subunits of protocatechuate 3 , 4-dioxygenase ( 3 , 4-PCD ( EC 1.13.11.3 ) ) were cloned from a Pseudomonas putida ( formerly P. aeruginosa ) ( ATCC 23975 ) genomic library prepared in lambda phage .
	manualset3
157150	2	410236	7	NULL	NULL	NULL	NULL	genomic library	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The genes that encode the alpha and beta subunits of protocatechuate 3 , 4-dioxygenase ( 3 , 4-PCD ( EC 1.13.11.3 ) ) were cloned from a Pseudomonas putida ( formerly P. aeruginosa ) ( ATCC 23975 ) genomic library prepared in lambda phage .
	manualset3
157152	3	410236	7	NULL	NULL	NULL	NULL	lambda phage	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The genes that encode the alpha and beta subunits of protocatechuate 3 , 4-dioxygenase ( 3 , 4-PCD ( EC 1.13.11.3 ) ) were cloned from a Pseudomonas putida ( formerly P. aeruginosa ) ( ATCC 23975 ) genomic library prepared in lambda phage .
	manualset3
157153	1	410237	7	NULL	NULL	0	NULL	suspension	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A suspension of the ear was performed using a strip of Marlex mesh .
	manualset3
157154	2	410237	7	NULL	NULL	0	NULL	ear	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A suspension of the ear was performed using a strip of Marlex mesh .
	manualset3
157155	3	410237	7	NULL	NULL	0	NULL	strip of Marlex mesh	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A suspension of the ear was performed using a strip of Marlex mesh .
	manualset3
157198	1	410238	7	NULL	NULL	0	NULL	genesis of any toxicological outcome	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The genesis of any toxicological or safety outcome is multifactorial and complex ; for this reason , it can be difficult for drug discovery projects to factor the avoidance of toxicity outcomes into their target design .
	manualset3
157199	2	410238	7	NULL	NULL	0	NULL	genesis of any safety outcome	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The genesis of any toxicological or safety outcome is multifactorial and complex ; for this reason , it can be difficult for drug discovery projects to factor the avoidance of toxicity outcomes into their target design .
	manualset3
157200	3	410238	7	NULL	NULL	0	NULL	drug discovery projects	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The genesis of any toxicological or safety outcome is multifactorial and complex ; for this reason , it can be difficult for drug discovery projects to factor the avoidance of toxicity outcomes into their target design .
	manualset3
157201	4	410238	7	NULL	NULL	0	NULL	factor	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The genesis of any toxicological or safety outcome is multifactorial and complex ; for this reason , it can be difficult for drug discovery projects to factor the avoidance of toxicity outcomes into their target design .
	manualset3
157202	5	410238	7	NULL	NULL	NULL	NULL	 toxicity outcomes	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The genesis of any toxicological or safety outcome is multifactorial and complex ; for this reason , it can be difficult for drug discovery projects to factor the avoidance of toxicity outcomes into their target design .
	manualset3
157203	6	410238	7	NULL	NULL	0	NULL	target design	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The genesis of any toxicological or safety outcome is multifactorial and complex ; for this reason , it can be difficult for drug discovery projects to factor the avoidance of toxicity outcomes into their target design .
	manualset3
157204	1	410239	7	NULL	NULL	NULL	NULL	genome	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The genome encodes nine antioxidant factors and nine phospholipases , which facilitate intracellular survival in phagocytes .
	manualset3
157205	2	410239	7	NULL	NULL	NULL	NULL	nine antioxidant factors	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The genome encodes nine antioxidant factors and nine phospholipases , which facilitate intracellular survival in phagocytes .
	manualset3
157206	3	410239	7	NULL	NULL	0	NULL	nine phospholipases	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The genome encodes nine antioxidant factors and nine phospholipases , which facilitate intracellular survival in phagocytes .
	manualset3
157207	4	410239	7	NULL	NULL	0	NULL	intracellular survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The genome encodes nine antioxidant factors and nine phospholipases , which facilitate intracellular survival in phagocytes .
	manualset3
157208	5	410239	7	NULL	NULL	0	NULL	phagocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The genome encodes nine antioxidant factors and nine phospholipases , which facilitate intracellular survival in phagocytes .
	manualset3
157209	1	410240	7	NULL	NULL	NULL	NULL	genome sequence	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The genome sequence of Haloferax volcanii is available and several comparative genomic in silico studies were performed that yielded novel insight for example into protein export , RNA modifications , small non-coding RNAs , and ubiquitin-like Small Archaeal Modifier Proteins .
	manualset3
157210	2	410240	7	NULL	NULL	0	NULL	 Haloferax volcanii	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The genome sequence of Haloferax volcanii is available and several comparative genomic in silico studies were performed that yielded novel insight for example into protein export , RNA modifications , small non-coding RNAs , and ubiquitin-like Small Archaeal Modifier Proteins .
	manualset3
157211	3	410240	7	NULL	NULL	0	NULL	comparative genomic in silico studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The genome sequence of Haloferax volcanii is available and several comparative genomic in silico studies were performed that yielded novel insight for example into protein export , RNA modifications , small non-coding RNAs , and ubiquitin-like Small Archaeal Modifier Proteins .
	manualset3
157212	4	410240	7	NULL	NULL	0	NULL	novel insight	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The genome sequence of Haloferax volcanii is available and several comparative genomic in silico studies were performed that yielded novel insight for example into protein export , RNA modifications , small non-coding RNAs , and ubiquitin-like Small Archaeal Modifier Proteins .
	manualset3
157213	5	410240	7	NULL	NULL	0	NULL	protein export	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The genome sequence of Haloferax volcanii is available and several comparative genomic in silico studies were performed that yielded novel insight for example into protein export , RNA modifications , small non-coding RNAs , and ubiquitin-like Small Archaeal Modifier Proteins .
	manualset3
157214	6	410240	7	NULL	NULL	0	NULL	RNA modifications	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The genome sequence of Haloferax volcanii is available and several comparative genomic in silico studies were performed that yielded novel insight for example into protein export , RNA modifications , small non-coding RNAs , and ubiquitin-like Small Archaeal Modifier Proteins .
	manualset3
157215	7	410240	7	NULL	NULL	0	NULL	small non-coding RNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The genome sequence of Haloferax volcanii is available and several comparative genomic in silico studies were performed that yielded novel insight for example into protein export , RNA modifications , small non-coding RNAs , and ubiquitin-like Small Archaeal Modifier Proteins .
	manualset3
157216	8	410240	7	NULL	NULL	NULL	NULL	ubiquitin-like Small Archaeal Modifier Proteins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The genome sequence of Haloferax volcanii is available and several comparative genomic in silico studies were performed that yielded novel insight for example into protein export , RNA modifications , small non-coding RNAs , and ubiquitin-like Small Archaeal Modifier Proteins .
	manualset3
157217	1	410241	7	NULL	NULL	NULL	NULL	genome structure	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The genome structure and gene heterogeneity were also consistent with the type of indigenous plasmids harbored by the strains .
	manualset3
157218	2	410241	7	NULL	NULL	0	NULL	gene heterogeneity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The genome structure and gene heterogeneity were also consistent with the type of indigenous plasmids harbored by the strains .
	manualset3
157219	3	410241	7	NULL	NULL	0	NULL	indigenous plasmids	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The genome structure and gene heterogeneity were also consistent with the type of indigenous plasmids harbored by the strains .
	manualset3
157220	4	410241	7	NULL	NULL	0	NULL	strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The genome structure and gene heterogeneity were also consistent with the type of indigenous plasmids harbored by the strains .
	manualset3
157221	1	410242	7	NULL	NULL	0	NULL	The genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The genome was predicted to encode small T antigen , large T antigen , and three capsid proteins : VP1 , VP2 , and VP3 .
	manualset3
157222	2	410242	7	NULL	NULL	0	NULL	small T antigen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The genome was predicted to encode small T antigen , large T antigen , and three capsid proteins : VP1 , VP2 , and VP3 .
	manualset3
157223	3	410242	7	NULL	NULL	0	NULL	large T antigen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The genome was predicted to encode small T antigen , large T antigen , and three capsid proteins : VP1 , VP2 , and VP3 .
	manualset3
157224	4	410242	7	NULL	NULL	0	NULL	three capsid proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The genome was predicted to encode small T antigen , large T antigen , and three capsid proteins : VP1 , VP2 , and VP3 .
	manualset3
157225	5	410242	7	NULL	NULL	0	NULL	VP1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The genome was predicted to encode small T antigen , large T antigen , and three capsid proteins : VP1 , VP2 , and VP3 .
	manualset3
157226	6	410242	7	NULL	NULL	0	NULL	VP2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The genome was predicted to encode small T antigen , large T antigen , and three capsid proteins : VP1 , VP2 , and VP3 .
	manualset3
157227	7	410242	7	NULL	NULL	0	NULL	VP3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The genome was predicted to encode small T antigen , large T antigen , and three capsid proteins : VP1 , VP2 , and VP3 .
	manualset3
157228	1	410243	7	NULL	NULL	NULL	NULL	genomic description 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The genomic description of this ETS/AP -1 - regulated , RAS-responsive , gene expression program provides a resource for understanding the role of these ETS factors in both an oncogenic setting and the developmental processes where these genes normally function .
	manualset3
157229	2	410243	7	NULL	NULL	NULL	NULL	RAS-responsive gene expression program	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The genomic description of this ETS/AP -1 - regulated , RAS-responsive , gene expression program provides a resource for understanding the role of these ETS factors in both an oncogenic setting and the developmental processes where these genes normally function .
	manualset3
157230	3	410243	7	NULL	NULL	0	NULL	gene expression program	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The genomic description of this ETS/AP -1 - regulated , RAS-responsive , gene expression program provides a resource for understanding the role of these ETS factors in both an oncogenic setting and the developmental processes where these genes normally function .
	manualset3
157231	4	410243	7	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The genomic description of this ETS/AP -1 - regulated , RAS-responsive , gene expression program provides a resource for understanding the role of these ETS factors in both an oncogenic setting and the developmental processes where these genes normally function .
	manualset3
157232	5	410243	7	NULL	NULL	NULL	NULL	ETS factors	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The genomic description of this ETS/AP -1 - regulated , RAS-responsive , gene expression program provides a resource for understanding the role of these ETS factors in both an oncogenic setting and the developmental processes where these genes normally function .
	manualset3
157233	6	410243	7	NULL	NULL	0	NULL	developmental processes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The genomic description of this ETS/AP -1 - regulated , RAS-responsive , gene expression program provides a resource for understanding the role of these ETS factors in both an oncogenic setting and the developmental processes where these genes normally function .
	manualset3
157234	7	410243	7	NULL	NULL	0	NULL	genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The genomic description of this ETS/AP -1 - regulated , RAS-responsive , gene expression program provides a resource for understanding the role of these ETS factors in both an oncogenic setting and the developmental processes where these genes normally function .
	manualset3
157338	9	410243	7	NULL	NULL	0	NULL	ETS/AP -1 - regulated gene expression program	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The genomic description of this ETS/AP -1 - regulated , RAS-responsive , gene expression program provides a resource for understanding the role of these ETS factors in both an oncogenic setting and the developmental processes where these genes normally function .
	manualset3
157339	10	410243	7	NULL	NULL	0	NULL	resource	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The genomic description of this ETS/AP -1 - regulated , RAS-responsive , gene expression program provides a resource for understanding the role of these ETS factors in both an oncogenic setting and the developmental processes where these genes normally function .
	manualset3
157340	11	410243	7	NULL	NULL	NULL	NULL	oncogenic setting	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The genomic description of this ETS/AP -1 - regulated , RAS-responsive , gene expression program provides a resource for understanding the role of these ETS factors in both an oncogenic setting and the developmental processes where these genes normally function .
	manualset3
157236	1	410244	7	NULL	NULL	0	NULL	genomic organization of a gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The genomic organization of a gene coding for an alpha 1 subunit of a voltage-gated calcium channel of Drosophila melanogaster ( Dmca IA ) was determined .
	manualset3
157237	2	410244	7	NULL	NULL	0	NULL	alpha 1 subunit 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The genomic organization of a gene coding for an alpha 1 subunit of a voltage-gated calcium channel of Drosophila melanogaster ( Dmca IA ) was determined .
	manualset3
157238	3	410244	7	NULL	NULL	0	NULL	voltage-gated calcium channel 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The genomic organization of a gene coding for an alpha 1 subunit of a voltage-gated calcium channel of Drosophila melanogaster ( Dmca IA ) was determined .
	manualset3
157239	4	410244	7	NULL	NULL	0	NULL	Drosophila melanogaster ( Dmca IA ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The genomic organization of a gene coding for an alpha 1 subunit of a voltage-gated calcium channel of Drosophila melanogaster ( Dmca IA ) was determined .
	manualset3
157240	1	410245	7	NULL	NULL	0	NULL	genomic organization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The genomic organization of the mRNAI and mRNAII 5 ' - untranslated sequences reveals that the mRNAs are encoded from two separate promoters which are 2.1 kbp apart on the single GGT gene .
	manualset3
157241	2	410245	7	NULL	NULL	NULL	NULL	mRNAI 5 ' - untranslated sequences	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The genomic organization of the mRNAI and mRNAII 5 ' - untranslated sequences reveals that the mRNAs are encoded from two separate promoters which are 2.1 kbp apart on the single GGT gene .
	manualset3
157242	3	410245	7	NULL	NULL	NULL	NULL	mRNAII 5 ' - untranslated sequences	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The genomic organization of the mRNAI and mRNAII 5 ' - untranslated sequences reveals that the mRNAs are encoded from two separate promoters which are 2.1 kbp apart on the single GGT gene .
	manualset3
157243	4	410245	7	NULL	NULL	0	NULL	mRNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The genomic organization of the mRNAI and mRNAII 5 ' - untranslated sequences reveals that the mRNAs are encoded from two separate promoters which are 2.1 kbp apart on the single GGT gene .
	manualset3
157244	5	410245	7	NULL	NULL	0	NULL	two separate promoters	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The genomic organization of the mRNAI and mRNAII 5 ' - untranslated sequences reveals that the mRNAs are encoded from two separate promoters which are 2.1 kbp apart on the single GGT gene .
	manualset3
157245	6	410245	7	NULL	NULL	0	NULL	2.1 kbp 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The genomic organization of the mRNAI and mRNAII 5 ' - untranslated sequences reveals that the mRNAs are encoded from two separate promoters which are 2.1 kbp apart on the single GGT gene .
	manualset3
157246	7	410245	7	NULL	NULL	0	NULL	single GGT gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The genomic organization of the mRNAI and mRNAII 5 ' - untranslated sequences reveals that the mRNAs are encoded from two separate promoters which are 2.1 kbp apart on the single GGT gene .
	manualset3
157247	1	410246	7	NULL	NULL	0	NULL	genotype distribution of 3 SNPs	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The genotype distribution of 3 SNPs differed between the IS and control subjects .
	manualset3
157248	2	410246	7	NULL	NULL	0	NULL	IS subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The genotype distribution of 3 SNPs differed between the IS and control subjects .
	manualset3
157249	3	410246	7	NULL	NULL	0	NULL	control subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The genotype distribution of 3 SNPs differed between the IS and control subjects .
	manualset3
157250	1	410247	7	NULL	NULL	NULL	NULL	geographical focus	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The geographical focus is on the United States .
	manualset3
157251	2	410247	7	NULL	NULL	0	NULL	United States	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The geographical focus is on the United States .
	manualset3
157252	1	410248	7	NULL	NULL	0	NULL	 geometries of vibrations	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The geometries and normal modes of vibrations obtained from ab initio HF and B3LYP/B3PW91 calculations are in good agreement with the experimentally observed data .
	manualset3
157253	2	410248	7	NULL	NULL	0	NULL	normal modes of vibrations	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The geometries and normal modes of vibrations obtained from ab initio HF and B3LYP/B3PW91 calculations are in good agreement with the experimentally observed data .
	manualset3
157254	3	410248	7	NULL	NULL	0	NULL	ab initio HF calculations	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The geometries and normal modes of vibrations obtained from ab initio HF and B3LYP/B3PW91 calculations are in good agreement with the experimentally observed data .
	manualset3
157255	4	410248	7	NULL	NULL	0	NULL	B3LYP/B3PW91 calculations	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The geometries and normal modes of vibrations obtained from ab initio HF and B3LYP/B3PW91 calculations are in good agreement with the experimentally observed data .
	manualset3
157256	5	410248	7	NULL	NULL	NULL	NULL	agreement	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The geometries and normal modes of vibrations obtained from ab initio HF and B3LYP/B3PW91 calculations are in good agreement with the experimentally observed data .
	manualset3
157257	6	410248	7	NULL	NULL	0	NULL	experimentally observed data	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The geometries and normal modes of vibrations obtained from ab initio HF and B3LYP/B3PW91 calculations are in good agreement with the experimentally observed data .
	manualset3
157266	1	410249	7	NULL	NULL	NULL	NULL	geometry of the dipropylene triamine ( dpt ) - Cu ( II ) end-group complexes 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The geometry of the dipropylene triamine ( dpt ) - Cu ( II ) end-group complexes for all dendrimer generations is reported for the first time and is found to be that of a square-based pyramid with each Cu ion bound to three nitrogen atoms ( Cu-N distance approximately 2.03 A ) of the dpt end group of the dendrimer .
	manualset3
157267	2	410249	7	NULL	NULL	0	NULL	first time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The geometry of the dipropylene triamine ( dpt ) - Cu ( II ) end-group complexes for all dendrimer generations is reported for the first time and is found to be that of a square-based pyramid with each Cu ion bound to three nitrogen atoms ( Cu-N distance approximately 2.03 A ) of the dpt end group of the dendrimer .
	manualset3
157268	3	410249	7	NULL	NULL	NULL	NULL	square-based pyramid with each Cu ion bound to three nitrogen atoms	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The geometry of the dipropylene triamine ( dpt ) - Cu ( II ) end-group complexes for all dendrimer generations is reported for the first time and is found to be that of a square-based pyramid with each Cu ion bound to three nitrogen atoms ( Cu-N distance approximately 2.03 A ) of the dpt end group of the dendrimer .
	manualset3
157269	4	410249	7	NULL	NULL	0	NULL	Cu-N distance approximately 2.03 A	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The geometry of the dipropylene triamine ( dpt ) - Cu ( II ) end-group complexes for all dendrimer generations is reported for the first time and is found to be that of a square-based pyramid with each Cu ion bound to three nitrogen atoms ( Cu-N distance approximately 2.03 A ) of the dpt end group of the dendrimer .
	manualset3
157270	5	410249	7	NULL	NULL	NULL	NULL	dpt end group of the dendrimer	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The geometry of the dipropylene triamine ( dpt ) - Cu ( II ) end-group complexes for all dendrimer generations is reported for the first time and is found to be that of a square-based pyramid with each Cu ion bound to three nitrogen atoms ( Cu-N distance approximately 2.03 A ) of the dpt end group of the dendrimer .
	manualset3
157272	6	410249	7	NULL	NULL	NULL	NULL	dendrimer generations	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The geometry of the dipropylene triamine ( dpt ) - Cu ( II ) end-group complexes for all dendrimer generations is reported for the first time and is found to be that of a square-based pyramid with each Cu ion bound to three nitrogen atoms ( Cu-N distance approximately 2.03 A ) of the dpt end group of the dendrimer .
	manualset3
157341	1	410250	7	NULL	NULL	NULL	NULL	protein	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The given protein proved to bind estradiol ( E2 ) with Ka of the 10 ( 7 ) M-1 order and possessed a rather marked hormonal affinity specificity .
	manualset3
157343	3	410250	7	NULL	NULL	0	NULL	estradiol ( E2 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The given protein proved to bind estradiol ( E2 ) with Ka of the 10 ( 7 ) M-1 order and possessed a rather marked hormonal affinity specificity .
	manualset3
157344	4	410250	7	NULL	NULL	0	NULL	Ka of the 10 ( 7 ) M-1 order	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The given protein proved to bind estradiol ( E2 ) with Ka of the 10 ( 7 ) M-1 order and possessed a rather marked hormonal affinity specificity .
	manualset3
157345	5	410250	7	NULL	NULL	NULL	NULL	hormonal affinity specificity	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The given protein proved to bind estradiol ( E2 ) with Ka of the 10 ( 7 ) M-1 order and possessed a rather marked hormonal affinity specificity .
	manualset3
157346	1	410251	7	NULL	NULL	0	NULL	synthetic DNA sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A synthetic DNA sequence coding for a soluble and flexible serine/glycine linker was then used to genetically fuse syncyt2Aa1 with the human single-chain antibody fragment ( scFv ) C6 .5 targeting p185 ( HER-2 ) , a cell-surface glycoprotein overexpressed in 30 % of human breast and ovarian cancers .
	manualset3
157347	2	410251	7	NULL	NULL	NULL	NULL	soluble serine/glycine linker 	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A synthetic DNA sequence coding for a soluble and flexible serine/glycine linker was then used to genetically fuse syncyt2Aa1 with the human single-chain antibody fragment ( scFv ) C6 .5 targeting p185 ( HER-2 ) , a cell-surface glycoprotein overexpressed in 30 % of human breast and ovarian cancers .
	manualset3
157348	3	410251	7	NULL	NULL	NULL	NULL	flexible serine/glycine linker	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A synthetic DNA sequence coding for a soluble and flexible serine/glycine linker was then used to genetically fuse syncyt2Aa1 with the human single-chain antibody fragment ( scFv ) C6 .5 targeting p185 ( HER-2 ) , a cell-surface glycoprotein overexpressed in 30 % of human breast and ovarian cancers .
	manualset3
157349	4	410251	7	NULL	NULL	0	NULL	fuse	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A synthetic DNA sequence coding for a soluble and flexible serine/glycine linker was then used to genetically fuse syncyt2Aa1 with the human single-chain antibody fragment ( scFv ) C6 .5 targeting p185 ( HER-2 ) , a cell-surface glycoprotein overexpressed in 30 % of human breast and ovarian cancers .
	manualset3
157350	5	410251	7	NULL	NULL	NULL	NULL	syncyt2Aa1	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A synthetic DNA sequence coding for a soluble and flexible serine/glycine linker was then used to genetically fuse syncyt2Aa1 with the human single-chain antibody fragment ( scFv ) C6 .5 targeting p185 ( HER-2 ) , a cell-surface glycoprotein overexpressed in 30 % of human breast and ovarian cancers .
	manualset3
157351	6	410251	7	NULL	NULL	0	NULL	human single-chain antibody fragment ( scFv ) C6 .5 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A synthetic DNA sequence coding for a soluble and flexible serine/glycine linker was then used to genetically fuse syncyt2Aa1 with the human single-chain antibody fragment ( scFv ) C6 .5 targeting p185 ( HER-2 ) , a cell-surface glycoprotein overexpressed in 30 % of human breast and ovarian cancers .
	manualset3
157352	7	410251	7	NULL	NULL	0	NULL	p185 ( HER-2 )	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A synthetic DNA sequence coding for a soluble and flexible serine/glycine linker was then used to genetically fuse syncyt2Aa1 with the human single-chain antibody fragment ( scFv ) C6 .5 targeting p185 ( HER-2 ) , a cell-surface glycoprotein overexpressed in 30 % of human breast and ovarian cancers .
	manualset3
157353	8	410251	7	NULL	NULL	0	NULL	cell-surface glycoprotein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A synthetic DNA sequence coding for a soluble and flexible serine/glycine linker was then used to genetically fuse syncyt2Aa1 with the human single-chain antibody fragment ( scFv ) C6 .5 targeting p185 ( HER-2 ) , a cell-surface glycoprotein overexpressed in 30 % of human breast and ovarian cancers .
	manualset3
157354	9	410251	7	NULL	NULL	0	NULL	30 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A synthetic DNA sequence coding for a soluble and flexible serine/glycine linker was then used to genetically fuse syncyt2Aa1 with the human single-chain antibody fragment ( scFv ) C6 .5 targeting p185 ( HER-2 ) , a cell-surface glycoprotein overexpressed in 30 % of human breast and ovarian cancers .
	manualset3
157355	10	410251	7	NULL	NULL	0	NULL	human breast cancer	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A synthetic DNA sequence coding for a soluble and flexible serine/glycine linker was then used to genetically fuse syncyt2Aa1 with the human single-chain antibody fragment ( scFv ) C6 .5 targeting p185 ( HER-2 ) , a cell-surface glycoprotein overexpressed in 30 % of human breast and ovarian cancers .
	manualset3
157356	11	410251	7	NULL	NULL	0	NULL	human ovarian cancers	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A synthetic DNA sequence coding for a soluble and flexible serine/glycine linker was then used to genetically fuse syncyt2Aa1 with the human single-chain antibody fragment ( scFv ) C6 .5 targeting p185 ( HER-2 ) , a cell-surface glycoprotein overexpressed in 30 % of human breast and ovarian cancers .
	manualset3
157357	1	410252	7	NULL	NULL	0	NULL	glassy carbon electrode	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The glassy carbon electrode was modified by the electrochemical reduction of a catechol para-substituted phenyldiazonium salt .
	manualset3
157358	2	410252	7	NULL	NULL	0	NULL	electrochemical reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The glassy carbon electrode was modified by the electrochemical reduction of a catechol para-substituted phenyldiazonium salt .
	manualset3
157359	3	410252	7	NULL	NULL	0	NULL	catechol para-substituted phenyldiazonium salt	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The glassy carbon electrode was modified by the electrochemical reduction of a catechol para-substituted phenyldiazonium salt .
	manualset3
157360	1	410253	7	NULL	NULL	0	NULL	globin chain	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The globin chain has 150 amino acid residues and a calculated Mr of 15 , 602.69 strongly suggesting that the amino terminus is acetylated .
	manualset3
157361	2	410253	7	NULL	NULL	0	NULL	150 amino acid residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The globin chain has 150 amino acid residues and a calculated Mr of 15 , 602.69 strongly suggesting that the amino terminus is acetylated .
	manualset3
157362	3	410253	7	NULL	NULL	0	NULL	Mr of 15 , 602.69	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The globin chain has 150 amino acid residues and a calculated Mr of 15 , 602.69 strongly suggesting that the amino terminus is acetylated .
	manualset3
157363	4	410253	7	NULL	NULL	NULL	NULL	amino terminus	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The globin chain has 150 amino acid residues and a calculated Mr of 15 , 602.69 strongly suggesting that the amino terminus is acetylated .
	manualset3
157364	1	410254	7	NULL	NULL	0	NULL	glomerulus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The glomerulus appeared to be contracted at three hours as well .
	manualset3
157365	2	410254	7	NULL	NULL	0	NULL	three hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The glomerulus appeared to be contracted at three hours as well .
	manualset3
157366	1	410255	7	NULL	NULL	NULL	NULL	glucoamylase inhibitor	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The glucoamylase inhibitor acarbose is a direct activator of phosphorylase kinase .
	manualset3
157367	2	410255	7	NULL	NULL	0	NULL	acarbose	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The glucoamylase inhibitor acarbose is a direct activator of phosphorylase kinase .
	manualset3
157369	3	410255	7	NULL	NULL	0	NULL	direct activator	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The glucoamylase inhibitor acarbose is a direct activator of phosphorylase kinase .
	manualset3
157370	4	410255	7	NULL	NULL	0	NULL	 phosphorylase kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The glucoamylase inhibitor acarbose is a direct activator of phosphorylase kinase .
	manualset3
157371	1	410256	7	NULL	NULL	NULL	NULL	glucose	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The glucose produced did not accumulate in the midgut lumen .
	manualset3
157373	2	410256	7	NULL	NULL	NULL	NULL	midgut lumen	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The glucose produced did not accumulate in the midgut lumen .
	manualset3
157374	1	410257	7	NULL	NULL	0	NULL	glucose	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The glucose self-infusion stimulated ingestion within 13-15 min in test 1 and produced a conditioned increase in licking that was apparent in the initial minute of tests 2 and 3 .
	manualset3
157375	2	410257	7	NULL	NULL	0	NULL	self-infusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The glucose self-infusion stimulated ingestion within 13-15 min in test 1 and produced a conditioned increase in licking that was apparent in the initial minute of tests 2 and 3 .
	manualset3
157376	3	410257	7	NULL	NULL	0	NULL	ingestion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The glucose self-infusion stimulated ingestion within 13-15 min in test 1 and produced a conditioned increase in licking that was apparent in the initial minute of tests 2 and 3 .
	manualset3
157377	4	410257	7	NULL	NULL	0	NULL	13-15 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The glucose self-infusion stimulated ingestion within 13-15 min in test 1 and produced a conditioned increase in licking that was apparent in the initial minute of tests 2 and 3 .
	manualset3
157378	5	410257	7	NULL	NULL	0	NULL	test 1	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The glucose self-infusion stimulated ingestion within 13-15 min in test 1 and produced a conditioned increase in licking that was apparent in the initial minute of tests 2 and 3 .
	manualset3
157379	6	410257	7	NULL	NULL	0	NULL	conditioned increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The glucose self-infusion stimulated ingestion within 13-15 min in test 1 and produced a conditioned increase in licking that was apparent in the initial minute of tests 2 and 3 .
	manualset3
157380	7	410257	7	NULL	NULL	NULL	NULL	 initial minute	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The glucose self-infusion stimulated ingestion within 13-15 min in test 1 and produced a conditioned increase in licking that was apparent in the initial minute of tests 2 and 3 .
	manualset3
157381	8	410257	7	NULL	NULL	NULL	NULL	tests 2	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The glucose self-infusion stimulated ingestion within 13-15 min in test 1 and produced a conditioned increase in licking that was apparent in the initial minute of tests 2 and 3 .
	manualset3
157382	9	410257	7	NULL	NULL	0	NULL	tests 3	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The glucose self-infusion stimulated ingestion within 13-15 min in test 1 and produced a conditioned increase in licking that was apparent in the initial minute of tests 2 and 3 .
	manualset3
157383	1	410258	7	NULL	NULL	0	NULL	glucosylation reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The glucosylation reaction was especially interesting for the production of valuable glucosides .
	manualset3
157384	2	410258	7	NULL	NULL	0	NULL	production 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The glucosylation reaction was especially interesting for the production of valuable glucosides .
	manualset3
157385	3	410258	7	NULL	NULL	0	NULL	valuable glucosides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The glucosylation reaction was especially interesting for the production of valuable glucosides .
	manualset3
157386	1	410259	7	NULL	NULL	0	NULL	glutamic acid content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The glutamic acid content decreased and arginine content increased as nitrate was provided to nitrogen-limited cells .
	manualset3
157387	2	410259	7	NULL	NULL	0	NULL	arginine content 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The glutamic acid content decreased and arginine content increased as nitrate was provided to nitrogen-limited cells .
	manualset3
157388	3	410259	7	NULL	NULL	0	NULL	nitrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The glutamic acid content decreased and arginine content increased as nitrate was provided to nitrogen-limited cells .
	manualset3
157389	4	410259	7	NULL	NULL	0	NULL	nitrogen-limited cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The glutamic acid content decreased and arginine content increased as nitrate was provided to nitrogen-limited cells .
	manualset3
157390	1	410260	7	NULL	NULL	NULL	NULL	glycine at position 61	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The glycine at position 61 was the only residue where no substitution was tolerated .
	manualset3
157391	2	410260	7	NULL	NULL	0	NULL	residue	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The glycine at position 61 was the only residue where no substitution was tolerated .
	manualset3
157392	3	410260	7	NULL	NULL	0	NULL	no substitution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The glycine at position 61 was the only residue where no substitution was tolerated .
	manualset3
157393	1	410261	7	NULL	NULL	0	NULL	goal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal is to show , and further predict , that supramolecular chemistry will continually increase its impact in organic synthetic methodology development .
	manualset3
157395	3	410261	7	NULL	NULL	0	NULL	predict	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal is to show , and further predict , that supramolecular chemistry will continually increase its impact in organic synthetic methodology development .
	manualset3
157396	4	410261	7	NULL	NULL	0	NULL	supramolecular chemistry	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal is to show , and further predict , that supramolecular chemistry will continually increase its impact in organic synthetic methodology development .
	manualset3
157398	6	410261	7	NULL	NULL	0	NULL	impact	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal is to show , and further predict , that supramolecular chemistry will continually increase its impact in organic synthetic methodology development .
	manualset3
157399	7	410261	7	NULL	NULL	NULL	NULL	organic synthetic methodology development	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The goal is to show , and further predict , that supramolecular chemistry will continually increase its impact in organic synthetic methodology development .
	manualset3
157401	1	410262	7	NULL	NULL	NULL	NULL	synthetic  site-directed mutagenesis study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A synthetic site-directed mutagenesis study of the non post-translationally modified silica precipitating R5 peptide reveals that the RRIL motif is critical in the formation of active silica precipitating assemblies .
	manualset3
157403	3	410262	7	NULL	NULL	0	NULL	non post-translationally modified silica precipitating R5 peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	A synthetic site-directed mutagenesis study of the non post-translationally modified silica precipitating R5 peptide reveals that the RRIL motif is critical in the formation of active silica precipitating assemblies .
	manualset3
157404	4	410262	7	NULL	NULL	0	NULL	RRIL motif	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A synthetic site-directed mutagenesis study of the non post-translationally modified silica precipitating R5 peptide reveals that the RRIL motif is critical in the formation of active silica precipitating assemblies .
	manualset3
157406	6	410262	7	NULL	NULL	0	NULL	formation of active silica precipitating assemblies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A synthetic site-directed mutagenesis study of the non post-translationally modified silica precipitating R5 peptide reveals that the RRIL motif is critical in the formation of active silica precipitating assemblies .
	manualset3
157407	1	410263	7	NULL	NULL	0	NULL	goal 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of applying epidemiological techniques to the study of occupational asthma is ultimately to identify more effective means to prevent its occurrence .
	manualset3
157408	2	410263	7	NULL	NULL	0	NULL	epidemiological techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of applying epidemiological techniques to the study of occupational asthma is ultimately to identify more effective means to prevent its occurrence .
	manualset3
157409	3	410263	7	NULL	NULL	NULL	NULL	study of occupational asthma	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The goal of applying epidemiological techniques to the study of occupational asthma is ultimately to identify more effective means to prevent its occurrence .
	manualset3
157411	5	410263	7	NULL	NULL	NULL	NULL	effective means	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The goal of applying epidemiological techniques to the study of occupational asthma is ultimately to identify more effective means to prevent its occurrence .
	manualset3
157413	7	410263	7	NULL	NULL	0	NULL	occurrence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of applying epidemiological techniques to the study of occupational asthma is ultimately to identify more effective means to prevent its occurrence .
	manualset3
157414	1	410264	7	NULL	NULL	0	NULL	goal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of given research was to define the role of morpho-functional changes in blood lymphocytes in the pathogenesis of psoriasis and the possibilities for their correction .
	manualset3
157415	2	410264	7	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of given research was to define the role of morpho-functional changes in blood lymphocytes in the pathogenesis of psoriasis and the possibilities for their correction .
	manualset3
157416	3	410264	7	NULL	NULL	NULL	NULL	morpho-functional changes	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The goal of given research was to define the role of morpho-functional changes in blood lymphocytes in the pathogenesis of psoriasis and the possibilities for their correction .
	manualset3
157417	4	410264	7	NULL	NULL	0	NULL	blood lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of given research was to define the role of morpho-functional changes in blood lymphocytes in the pathogenesis of psoriasis and the possibilities for their correction .
	manualset3
157418	5	410264	7	NULL	NULL	0	NULL	 pathogenesis of psoriasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of given research was to define the role of morpho-functional changes in blood lymphocytes in the pathogenesis of psoriasis and the possibilities for their correction .
	manualset3
157419	6	410264	7	NULL	NULL	NULL	NULL	correction	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The goal of given research was to define the role of morpho-functional changes in blood lymphocytes in the pathogenesis of psoriasis and the possibilities for their correction .
	manualset3
158398	7	410264	7	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of given research was to define the role of morpho-functional changes in blood lymphocytes in the pathogenesis of psoriasis and the possibilities for their correction .
	manualset3
159036	8	410264	7	NULL	NULL	0	NULL	possibilities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of given research was to define the role of morpho-functional changes in blood lymphocytes in the pathogenesis of psoriasis and the possibilities for their correction .
	manualset3
157420	1	410265	7	NULL	NULL	NULL	NULL	goal	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The goal of our article is to describe new possibilities of radiotherapy , including neoadjuvant and adjuvant setting , intraoperative radiotherapy , interstitial brachytherapy and the combination with surgery .
	manualset3
157421	2	410265	7	NULL	NULL	0	NULL	new possibilities of radiotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of our article is to describe new possibilities of radiotherapy , including neoadjuvant and adjuvant setting , intraoperative radiotherapy , interstitial brachytherapy and the combination with surgery .
	manualset3
157422	3	410265	7	NULL	NULL	0	NULL	neoadjuvant setting	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of our article is to describe new possibilities of radiotherapy , including neoadjuvant and adjuvant setting , intraoperative radiotherapy , interstitial brachytherapy and the combination with surgery .
	manualset3
157423	4	410265	7	NULL	NULL	0	NULL	adjuvant setting	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of our article is to describe new possibilities of radiotherapy , including neoadjuvant and adjuvant setting , intraoperative radiotherapy , interstitial brachytherapy and the combination with surgery .
	manualset3
157424	5	410265	7	NULL	NULL	0	NULL	intraoperative radiotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of our article is to describe new possibilities of radiotherapy , including neoadjuvant and adjuvant setting , intraoperative radiotherapy , interstitial brachytherapy and the combination with surgery .
	manualset3
157425	6	410265	7	NULL	NULL	0	NULL	interstitial brachytherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of our article is to describe new possibilities of radiotherapy , including neoadjuvant and adjuvant setting , intraoperative radiotherapy , interstitial brachytherapy and the combination with surgery .
	manualset3
157426	7	410265	7	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of our article is to describe new possibilities of radiotherapy , including neoadjuvant and adjuvant setting , intraoperative radiotherapy , interstitial brachytherapy and the combination with surgery .
	manualset3
157445	8	410265	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of our article is to describe new possibilities of radiotherapy , including neoadjuvant and adjuvant setting , intraoperative radiotherapy , interstitial brachytherapy and the combination with surgery .
	manualset3
159037	9	410265	7	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of our article is to describe new possibilities of radiotherapy , including neoadjuvant and adjuvant setting , intraoperative radiotherapy , interstitial brachytherapy and the combination with surgery .
	manualset3
157427	1	410266	7	NULL	NULL	0	NULL	goal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of the study was the evaluation of the role of the following nuclear antibodies : anti-Ro ( SS-A ) , anti-La ( SS-B ) and anti-Sm in the endothelium damage process in the SLE patients with symptoms of microcirculation disturbances .
	manualset3
157428	2	410266	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of the study was the evaluation of the role of the following nuclear antibodies : anti-Ro ( SS-A ) , anti-La ( SS-B ) and anti-Sm in the endothelium damage process in the SLE patients with symptoms of microcirculation disturbances .
	manualset3
157429	3	410266	7	NULL	NULL	0	NULL	evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of the study was the evaluation of the role of the following nuclear antibodies : anti-Ro ( SS-A ) , anti-La ( SS-B ) and anti-Sm in the endothelium damage process in the SLE patients with symptoms of microcirculation disturbances .
	manualset3
157430	4	410266	7	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of the study was the evaluation of the role of the following nuclear antibodies : anti-Ro ( SS-A ) , anti-La ( SS-B ) and anti-Sm in the endothelium damage process in the SLE patients with symptoms of microcirculation disturbances .
	manualset3
157431	5	410266	7	NULL	NULL	NULL	NULL	nuclear antibodies	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The goal of the study was the evaluation of the role of the following nuclear antibodies : anti-Ro ( SS-A ) , anti-La ( SS-B ) and anti-Sm in the endothelium damage process in the SLE patients with symptoms of microcirculation disturbances .
	manualset3
157432	6	410266	7	NULL	NULL	0	NULL	anti-Ro ( SS-A ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of the study was the evaluation of the role of the following nuclear antibodies : anti-Ro ( SS-A ) , anti-La ( SS-B ) and anti-Sm in the endothelium damage process in the SLE patients with symptoms of microcirculation disturbances .
	manualset3
157433	7	410266	7	NULL	NULL	0	NULL	anti-La ( SS-B )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of the study was the evaluation of the role of the following nuclear antibodies : anti-Ro ( SS-A ) , anti-La ( SS-B ) and anti-Sm in the endothelium damage process in the SLE patients with symptoms of microcirculation disturbances .
	manualset3
157434	8	410266	7	NULL	NULL	0	NULL	anti-Sm	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of the study was the evaluation of the role of the following nuclear antibodies : anti-Ro ( SS-A ) , anti-La ( SS-B ) and anti-Sm in the endothelium damage process in the SLE patients with symptoms of microcirculation disturbances .
	manualset3
157435	9	410266	7	NULL	NULL	0	NULL	endothelium damage process	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of the study was the evaluation of the role of the following nuclear antibodies : anti-Ro ( SS-A ) , anti-La ( SS-B ) and anti-Sm in the endothelium damage process in the SLE patients with symptoms of microcirculation disturbances .
	manualset3
157436	10	410266	7	NULL	NULL	0	NULL	SLE patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of the study was the evaluation of the role of the following nuclear antibodies : anti-Ro ( SS-A ) , anti-La ( SS-B ) and anti-Sm in the endothelium damage process in the SLE patients with symptoms of microcirculation disturbances .
	manualset3
157437	11	410266	7	NULL	NULL	0	NULL	symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of the study was the evaluation of the role of the following nuclear antibodies : anti-Ro ( SS-A ) , anti-La ( SS-B ) and anti-Sm in the endothelium damage process in the SLE patients with symptoms of microcirculation disturbances .
	manualset3
157438	12	410266	7	NULL	NULL	0	NULL	microcirculation disturbances	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of the study was the evaluation of the role of the following nuclear antibodies : anti-Ro ( SS-A ) , anti-La ( SS-B ) and anti-Sm in the endothelium damage process in the SLE patients with symptoms of microcirculation disturbances .
	manualset3
157439	1	410267	7	NULL	NULL	NULL	NULL	goal 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The goal of this review is to highlight some of the changes in mitochondrial proteomic make-up that are associated with the development of HF in an effort to identify target axes and candidate proteins contributing to disease development .
	manualset3
157440	2	410267	7	NULL	NULL	NULL	NULL	mitochondrial proteomic make-up	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The goal of this review is to highlight some of the changes in mitochondrial proteomic make-up that are associated with the development of HF in an effort to identify target axes and candidate proteins contributing to disease development .
	manualset3
157441	3	410267	7	NULL	NULL	0	NULL	development of HF	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of this review is to highlight some of the changes in mitochondrial proteomic make-up that are associated with the development of HF in an effort to identify target axes and candidate proteins contributing to disease development .
	manualset3
157442	4	410267	7	NULL	NULL	0	NULL	 target axes	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of this review is to highlight some of the changes in mitochondrial proteomic make-up that are associated with the development of HF in an effort to identify target axes and candidate proteins contributing to disease development .
	manualset3
157443	5	410267	7	NULL	NULL	0	NULL	candidate proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of this review is to highlight some of the changes in mitochondrial proteomic make-up that are associated with the development of HF in an effort to identify target axes and candidate proteins contributing to disease development .
	manualset3
157444	6	410267	7	NULL	NULL	0	NULL	disease development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of this review is to highlight some of the changes in mitochondrial proteomic make-up that are associated with the development of HF in an effort to identify target axes and candidate proteins contributing to disease development .
	manualset3
157446	7	410267	7	NULL	NULL	0	NULL	review	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of this review is to highlight some of the changes in mitochondrial proteomic make-up that are associated with the development of HF in an effort to identify target axes and candidate proteins contributing to disease development .
	manualset3
157447	1	410268	7	NULL	NULL	0	NULL	goal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of this study was to examine the relationship between suicide and violence against others in patients with major psychiatric disorders and to compare psychiatric symptoms associated with suicide in violent and non-violent patients .
	manualset3
157448	2	410268	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of this study was to examine the relationship between suicide and violence against others in patients with major psychiatric disorders and to compare psychiatric symptoms associated with suicide in violent and non-violent patients .
	manualset3
157449	3	410268	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of this study was to examine the relationship between suicide and violence against others in patients with major psychiatric disorders and to compare psychiatric symptoms associated with suicide in violent and non-violent patients .
	manualset3
157450	4	410268	7	NULL	NULL	0	NULL	suicide	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of this study was to examine the relationship between suicide and violence against others in patients with major psychiatric disorders and to compare psychiatric symptoms associated with suicide in violent and non-violent patients .
	manualset3
157451	5	410268	7	NULL	NULL	0	NULL	violence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of this study was to examine the relationship between suicide and violence against others in patients with major psychiatric disorders and to compare psychiatric symptoms associated with suicide in violent and non-violent patients .
	manualset3
157452	6	410268	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of this study was to examine the relationship between suicide and violence against others in patients with major psychiatric disorders and to compare psychiatric symptoms associated with suicide in violent and non-violent patients .
	manualset3
157453	7	410268	7	NULL	NULL	0	NULL	major psychiatric disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of this study was to examine the relationship between suicide and violence against others in patients with major psychiatric disorders and to compare psychiatric symptoms associated with suicide in violent and non-violent patients .
	manualset3
157454	8	410268	7	NULL	NULL	0	NULL	psychiatric symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of this study was to examine the relationship between suicide and violence against others in patients with major psychiatric disorders and to compare psychiatric symptoms associated with suicide in violent and non-violent patients .
	manualset3
157455	9	410268	7	NULL	NULL	0	NULL	suicide	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of this study was to examine the relationship between suicide and violence against others in patients with major psychiatric disorders and to compare psychiatric symptoms associated with suicide in violent and non-violent patients .
	manualset3
157456	10	410268	7	NULL	NULL	NULL	NULL	 violent patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The goal of this study was to examine the relationship between suicide and violence against others in patients with major psychiatric disorders and to compare psychiatric symptoms associated with suicide in violent and non-violent patients .
	manualset3
158399	11	410268	7	NULL	NULL	0	NULL	non-violent patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of this study was to examine the relationship between suicide and violence against others in patients with major psychiatric disorders and to compare psychiatric symptoms associated with suicide in violent and non-violent patients .
	manualset3
157457	1	410269	7	NULL	NULL	0	NULL	goal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of this work was to create a model for the long persistence of Mycoplasma gallisepticum in depleted medium and under low growth temperature followed by proteomic study of the model .
	manualset3
157458	2	410269	7	NULL	NULL	0	NULL	work	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of this work was to create a model for the long persistence of Mycoplasma gallisepticum in depleted medium and under low growth temperature followed by proteomic study of the model .
	manualset3
157459	3	410269	7	NULL	NULL	0	NULL	model 	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of this work was to create a model for the long persistence of Mycoplasma gallisepticum in depleted medium and under low growth temperature followed by proteomic study of the model .
	manualset3
157460	4	410269	7	NULL	NULL	NULL	NULL	Mycoplasma gallisepticum	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The goal of this work was to create a model for the long persistence of Mycoplasma gallisepticum in depleted medium and under low growth temperature followed by proteomic study of the model .
	manualset3
157461	5	410269	7	NULL	NULL	0	NULL	low growth temperature	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of this work was to create a model for the long persistence of Mycoplasma gallisepticum in depleted medium and under low growth temperature followed by proteomic study of the model .
	manualset3
157462	6	410269	7	NULL	NULL	0	NULL	proteomic study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of this work was to create a model for the long persistence of Mycoplasma gallisepticum in depleted medium and under low growth temperature followed by proteomic study of the model .
	manualset3
157463	7	410269	7	NULL	NULL	0	NULL	model	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of this work was to create a model for the long persistence of Mycoplasma gallisepticum in depleted medium and under low growth temperature followed by proteomic study of the model .
	manualset3
157464	8	410269	7	NULL	NULL	NULL	NULL	depleted medium 	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The goal of this work was to create a model for the long persistence of Mycoplasma gallisepticum in depleted medium and under low growth temperature followed by proteomic study of the model .
	manualset3
157465	1	410270	7	NULL	NULL	0	NULL	goal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of this work was to develop penalized maximum likelihood ( PML ) algorithms for a novel cross-tracer prior that exploits the fact that the two images reconstructed from simultaneous dual-isotope MPS projection data are perfectly registered in space .
	manualset3
157466	2	410270	7	NULL	NULL	0	NULL	work	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of this work was to develop penalized maximum likelihood ( PML ) algorithms for a novel cross-tracer prior that exploits the fact that the two images reconstructed from simultaneous dual-isotope MPS projection data are perfectly registered in space .
	manualset3
157467	3	410270	7	NULL	NULL	0	NULL	penalized maximum likelihood ( PML ) algorithms	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of this work was to develop penalized maximum likelihood ( PML ) algorithms for a novel cross-tracer prior that exploits the fact that the two images reconstructed from simultaneous dual-isotope MPS projection data are perfectly registered in space .
	manualset3
157468	4	410270	7	NULL	NULL	0	NULL	novel cross-tracer	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of this work was to develop penalized maximum likelihood ( PML ) algorithms for a novel cross-tracer prior that exploits the fact that the two images reconstructed from simultaneous dual-isotope MPS projection data are perfectly registered in space .
	manualset3
157469	5	410270	7	NULL	NULL	0	NULL	two images	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of this work was to develop penalized maximum likelihood ( PML ) algorithms for a novel cross-tracer prior that exploits the fact that the two images reconstructed from simultaneous dual-isotope MPS projection data are perfectly registered in space .
	manualset3
157470	6	410270	7	NULL	NULL	0	NULL	dual-isotope MPS projection data 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of this work was to develop penalized maximum likelihood ( PML ) algorithms for a novel cross-tracer prior that exploits the fact that the two images reconstructed from simultaneous dual-isotope MPS projection data are perfectly registered in space .
	manualset3
157471	7	410270	7	NULL	NULL	0	NULL	 space	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The goal of this work was to develop penalized maximum likelihood ( PML ) algorithms for a novel cross-tracer prior that exploits the fact that the two images reconstructed from simultaneous dual-isotope MPS projection data are perfectly registered in space .
	manualset3
157472	1	410271	7	NULL	NULL	0	NULL	goals	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The goals of therapy in managing asthma in a pregnant women are identical to those in a nonpregnant woman with asthma .
	manualset3
157473	2	410271	7	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The goals of therapy in managing asthma in a pregnant women are identical to those in a nonpregnant woman with asthma .
	manualset3
157474	3	410271	7	NULL	NULL	0	NULL	asthma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The goals of therapy in managing asthma in a pregnant women are identical to those in a nonpregnant woman with asthma .
	manualset3
157475	4	410271	7	NULL	NULL	0	NULL	pregnant women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The goals of therapy in managing asthma in a pregnant women are identical to those in a nonpregnant woman with asthma .
	manualset3
157476	5	410271	7	NULL	NULL	0	NULL	nonpregnant woman	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The goals of therapy in managing asthma in a pregnant women are identical to those in a nonpregnant woman with asthma .
	manualset3
157477	6	410271	7	NULL	NULL	0	NULL	asthma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The goals of therapy in managing asthma in a pregnant women are identical to those in a nonpregnant woman with asthma .
	manualset3
157478	1	410272	7	NULL	NULL	0	NULL	gold standard dermatologic agent 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The gold standard dermatologic agent for skin lightening was hydroquinone , until regulatory agencies in Japan , Europe , and most recently in the United States questioned the safety of this substance .
	manualset3
157479	2	410272	7	NULL	NULL	0	NULL	hydroquinone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The gold standard dermatologic agent for skin lightening was hydroquinone , until regulatory agencies in Japan , Europe , and most recently in the United States questioned the safety of this substance .
	manualset3
157480	3	410272	7	NULL	NULL	NULL	NULL	agencies	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The gold standard dermatologic agent for skin lightening was hydroquinone , until regulatory agencies in Japan , Europe , and most recently in the United States questioned the safety of this substance .
	manualset3
157481	4	410272	7	NULL	NULL	0	NULL	Japan	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The gold standard dermatologic agent for skin lightening was hydroquinone , until regulatory agencies in Japan , Europe , and most recently in the United States questioned the safety of this substance .
	manualset3
157482	5	410272	7	NULL	NULL	0	NULL	Europe	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The gold standard dermatologic agent for skin lightening was hydroquinone , until regulatory agencies in Japan , Europe , and most recently in the United States questioned the safety of this substance .
	manualset3
157483	6	410272	7	NULL	NULL	0	NULL	United States	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The gold standard dermatologic agent for skin lightening was hydroquinone , until regulatory agencies in Japan , Europe , and most recently in the United States questioned the safety of this substance .
	manualset3
157484	7	410272	7	NULL	NULL	0	NULL	substance	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The gold standard dermatologic agent for skin lightening was hydroquinone , until regulatory agencies in Japan , Europe , and most recently in the United States questioned the safety of this substance .
	manualset3
158509	8	410272	7	NULL	NULL	0	NULL	skin lightening	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The gold standard dermatologic agent for skin lightening was hydroquinone , until regulatory agencies in Japan , Europe , and most recently in the United States questioned the safety of this substance .
	manualset3
157485	1	410273	7	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The good correlation between the amount of charge underlying the presteady-state currents and the transport-associated current indicates that both processes are due to the activity of the transporter .
	manualset3
157486	2	410273	7	NULL	NULL	0	NULL	 charge	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The good correlation between the amount of charge underlying the presteady-state currents and the transport-associated current indicates that both processes are due to the activity of the transporter .
	manualset3
157487	3	410273	7	NULL	NULL	0	NULL	 presteady-state currents	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The good correlation between the amount of charge underlying the presteady-state currents and the transport-associated current indicates that both processes are due to the activity of the transporter .
	manualset3
157488	4	410273	7	NULL	NULL	0	NULL	transport-associated current	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The good correlation between the amount of charge underlying the presteady-state currents and the transport-associated current indicates that both processes are due to the activity of the transporter .
	manualset3
157489	5	410273	7	NULL	NULL	0	NULL	transporter	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The good correlation between the amount of charge underlying the presteady-state currents and the transport-associated current indicates that both processes are due to the activity of the transporter .
	manualset3
157496	6	410273	7	NULL	NULL	0	NULL	processes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The good correlation between the amount of charge underlying the presteady-state currents and the transport-associated current indicates that both processes are due to the activity of the transporter .
	manualset3
157497	7	410273	7	NULL	NULL	0	NULL	activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The good correlation between the amount of charge underlying the presteady-state currents and the transport-associated current indicates that both processes are due to the activity of the transporter .
	manualset3
157498	1	410274	7	NULL	NULL	0	NULL	SAC clinkers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The good quality SAC clinkers are obtained by controlling the compositional parameters at alkalinity modulus ( C ( m ) ) around 1.05 , alumina-sulfur ratio ( P ) around 2.5 , alumina-silica ratio ( N ) around 2.0 ~ 3.0 and firing the raw mixes at 1250 C for 2h .
	manualset3
157499	2	410274	7	NULL	NULL	0	NULL	compositional parameters	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The good quality SAC clinkers are obtained by controlling the compositional parameters at alkalinity modulus ( C ( m ) ) around 1.05 , alumina-sulfur ratio ( P ) around 2.5 , alumina-silica ratio ( N ) around 2.0 ~ 3.0 and firing the raw mixes at 1250 C for 2h .
	manualset3
157500	3	410274	7	NULL	NULL	NULL	NULL	 alkalinity modulus ( C ( m ) )	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The good quality SAC clinkers are obtained by controlling the compositional parameters at alkalinity modulus ( C ( m ) ) around 1.05 , alumina-sulfur ratio ( P ) around 2.5 , alumina-silica ratio ( N ) around 2.0 ~ 3.0 and firing the raw mixes at 1250 C for 2h .
	manualset3
157501	4	410274	7	NULL	NULL	0	NULL	1.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The good quality SAC clinkers are obtained by controlling the compositional parameters at alkalinity modulus ( C ( m ) ) around 1.05 , alumina-sulfur ratio ( P ) around 2.5 , alumina-silica ratio ( N ) around 2.0 ~ 3.0 and firing the raw mixes at 1250 C for 2h .
	manualset3
157502	5	410274	7	NULL	NULL	NULL	NULL	alumina-sulfur ratio ( P )	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The good quality SAC clinkers are obtained by controlling the compositional parameters at alkalinity modulus ( C ( m ) ) around 1.05 , alumina-sulfur ratio ( P ) around 2.5 , alumina-silica ratio ( N ) around 2.0 ~ 3.0 and firing the raw mixes at 1250 C for 2h .
	manualset3
157503	6	410274	7	NULL	NULL	0	NULL	 2.5	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The good quality SAC clinkers are obtained by controlling the compositional parameters at alkalinity modulus ( C ( m ) ) around 1.05 , alumina-sulfur ratio ( P ) around 2.5 , alumina-silica ratio ( N ) around 2.0 ~ 3.0 and firing the raw mixes at 1250 C for 2h .
	manualset3
157504	7	410274	7	NULL	NULL	0	NULL	alumina-silica ratio ( N )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The good quality SAC clinkers are obtained by controlling the compositional parameters at alkalinity modulus ( C ( m ) ) around 1.05 , alumina-sulfur ratio ( P ) around 2.5 , alumina-silica ratio ( N ) around 2.0 ~ 3.0 and firing the raw mixes at 1250 C for 2h .
	manualset3
157505	8	410274	7	NULL	NULL	0	NULL	2.0 ~ 3.0	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The good quality SAC clinkers are obtained by controlling the compositional parameters at alkalinity modulus ( C ( m ) ) around 1.05 , alumina-sulfur ratio ( P ) around 2.5 , alumina-silica ratio ( N ) around 2.0 ~ 3.0 and firing the raw mixes at 1250 C for 2h .
	manualset3
157506	9	410274	7	NULL	NULL	0	NULL	raw mixes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The good quality SAC clinkers are obtained by controlling the compositional parameters at alkalinity modulus ( C ( m ) ) around 1.05 , alumina-sulfur ratio ( P ) around 2.5 , alumina-silica ratio ( N ) around 2.0 ~ 3.0 and firing the raw mixes at 1250 C for 2h .
	manualset3
157507	10	410274	7	NULL	NULL	0	NULL	1250 C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The good quality SAC clinkers are obtained by controlling the compositional parameters at alkalinity modulus ( C ( m ) ) around 1.05 , alumina-sulfur ratio ( P ) around 2.5 , alumina-silica ratio ( N ) around 2.0 ~ 3.0 and firing the raw mixes at 1250 C for 2h .
	manualset3
157508	11	410274	7	NULL	NULL	0	NULL	2h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The good quality SAC clinkers are obtained by controlling the compositional parameters at alkalinity modulus ( C ( m ) ) around 1.05 , alumina-sulfur ratio ( P ) around 2.5 , alumina-silica ratio ( N ) around 2.0 ~ 3.0 and firing the raw mixes at 1250 C for 2h .
	manualset3
157509	1	410275	7	NULL	NULL	0	NULL	government	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The government attempted to stay out of the debate at first .
	manualset3
157510	2	410275	7	NULL	NULL	NULL	NULL	debate	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The government attempted to stay out of the debate at first .
	manualset3
157512	1	410276	7	NULL	NULL	0	NULL	government 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The government is focusing on the appropriation of funds to support family planning programs in order not to find itself flatfooted if foreign funders decide to withdraw their support within 5 years .
	manualset3
157513	2	410276	7	NULL	NULL	0	NULL	appropriation of funds	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The government is focusing on the appropriation of funds to support family planning programs in order not to find itself flatfooted if foreign funders decide to withdraw their support within 5 years .
	manualset3
157514	3	410276	7	NULL	NULL	0	NULL	family planning programs	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The government is focusing on the appropriation of funds to support family planning programs in order not to find itself flatfooted if foreign funders decide to withdraw their support within 5 years .
	manualset3
157516	5	410276	7	NULL	NULL	0	NULL	foreign funders	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The government is focusing on the appropriation of funds to support family planning programs in order not to find itself flatfooted if foreign funders decide to withdraw their support within 5 years .
	manualset3
157517	6	410276	7	NULL	NULL	0	NULL	support 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The government is focusing on the appropriation of funds to support family planning programs in order not to find itself flatfooted if foreign funders decide to withdraw their support within 5 years .
	manualset3
157518	7	410276	7	NULL	NULL	0	NULL	5 years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The government is focusing on the appropriation of funds to support family planning programs in order not to find itself flatfooted if foreign funders decide to withdraw their support within 5 years .
	manualset3
157519	1	410277	7	NULL	NULL	0	NULL	 grade factor 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The grade factor did not effect the survival rate significantly .
	manualset3
157521	2	410277	7	NULL	NULL	NULL	NULL	survival rate	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The grade factor did not effect the survival rate significantly .
	manualset3
157522	1	410278	7	NULL	NULL	NULL	NULL	 graded-index profiles	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The graded-index profiles of the optical fibers are almost the same as those of the corresponding preforms with cladding sheaths .
	manualset3
157523	2	410278	7	NULL	NULL	NULL	NULL	optical fibers	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The graded-index profiles of the optical fibers are almost the same as those of the corresponding preforms with cladding sheaths .
	manualset3
157524	3	410278	7	NULL	NULL	NULL	NULL	cladding sheaths	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The graded-index profiles of the optical fibers are almost the same as those of the corresponding preforms with cladding sheaths .
	manualset3
157525	4	410278	7	NULL	NULL	NULL	NULL	preforms	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The graded-index profiles of the optical fibers are almost the same as those of the corresponding preforms with cladding sheaths .
	manualset3
157526	1	410279	7	NULL	NULL	0	NULL	granuloma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The granuloma was located in the central part of the tongue and appeared dark pink in color .
	manualset3
157527	2	410279	7	NULL	NULL	0	NULL	central part of the tongue 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The granuloma was located in the central part of the tongue and appeared dark pink in color .
	manualset3
157528	3	410279	7	NULL	NULL	0	NULL	color	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The granuloma was located in the central part of the tongue and appeared dark pink in color .
	manualset3
157529	1	410280	7	NULL	NULL	0	NULL	great impact 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The great impact in public health of the dysfunction of protective serum proteins requires individual clinical recognition , appropriate preventive measures , and delineation of management , including with anti-inflammatory drugs .
	manualset3
157530	2	410280	7	NULL	NULL	0	NULL	public health	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The great impact in public health of the dysfunction of protective serum proteins requires individual clinical recognition , appropriate preventive measures , and delineation of management , including with anti-inflammatory drugs .
	manualset3
157531	3	410280	7	NULL	NULL	NULL	NULL	dysfunction	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The great impact in public health of the dysfunction of protective serum proteins requires individual clinical recognition , appropriate preventive measures , and delineation of management , including with anti-inflammatory drugs .
	manualset3
157532	4	410280	7	NULL	NULL	0	NULL	protective serum proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The great impact in public health of the dysfunction of protective serum proteins requires individual clinical recognition , appropriate preventive measures , and delineation of management , including with anti-inflammatory drugs .
	manualset3
157533	5	410280	7	NULL	NULL	0	NULL	clinical recognition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The great impact in public health of the dysfunction of protective serum proteins requires individual clinical recognition , appropriate preventive measures , and delineation of management , including with anti-inflammatory drugs .
	manualset3
157534	6	410280	7	NULL	NULL	0	NULL	preventive measures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The great impact in public health of the dysfunction of protective serum proteins requires individual clinical recognition , appropriate preventive measures , and delineation of management , including with anti-inflammatory drugs .
	manualset3
157535	7	410280	7	NULL	NULL	0	NULL	delineation of management 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The great impact in public health of the dysfunction of protective serum proteins requires individual clinical recognition , appropriate preventive measures , and delineation of management , including with anti-inflammatory drugs .
	manualset3
157536	8	410280	7	NULL	NULL	0	NULL	anti-inflammatory drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The great impact in public health of the dysfunction of protective serum proteins requires individual clinical recognition , appropriate preventive measures , and delineation of management , including with anti-inflammatory drugs .
	manualset3
157537	1	410281	7	NULL	NULL	0	NULL	great technical facility	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The great technical facility of operations of musculo-aponeurotic transposition , has led surgeons to discard plastic operations on the ligaments .
	manualset3
157538	2	410281	7	NULL	NULL	0	NULL	operations 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The great technical facility of operations of musculo-aponeurotic transposition , has led surgeons to discard plastic operations on the ligaments .
	manualset3
157539	3	410281	7	NULL	NULL	NULL	NULL	musculo-aponeurotic transposition	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The great technical facility of operations of musculo-aponeurotic transposition , has led surgeons to discard plastic operations on the ligaments .
	manualset3
157540	4	410281	7	NULL	NULL	0	NULL	surgeons	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The great technical facility of operations of musculo-aponeurotic transposition , has led surgeons to discard plastic operations on the ligaments .
	manualset3
157541	5	410281	7	NULL	NULL	0	NULL	plastic operations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The great technical facility of operations of musculo-aponeurotic transposition , has led surgeons to discard plastic operations on the ligaments .
	manualset3
157542	6	410281	7	NULL	NULL	0	NULL	 ligaments	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The great technical facility of operations of musculo-aponeurotic transposition , has led surgeons to discard plastic operations on the ligaments .
	manualset3
157543	1	410282	7	NULL	NULL	0	NULL	greater number of histidines	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The greater number of histidines and the greater strength of ligation are expected to slow conversion of the histidine-misligated forms to the obligatory aquo-heme intermediate during the ligand exchange phase of folding .
	manualset3
157544	2	410282	7	NULL	NULL	0	NULL	greater strength of ligation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The greater number of histidines and the greater strength of ligation are expected to slow conversion of the histidine-misligated forms to the obligatory aquo-heme intermediate during the ligand exchange phase of folding .
	manualset3
157545	3	410282	7	NULL	NULL	0	NULL	conversion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The greater number of histidines and the greater strength of ligation are expected to slow conversion of the histidine-misligated forms to the obligatory aquo-heme intermediate during the ligand exchange phase of folding .
	manualset3
157546	4	410282	7	NULL	NULL	NULL	NULL	histidine-misligated forms	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The greater number of histidines and the greater strength of ligation are expected to slow conversion of the histidine-misligated forms to the obligatory aquo-heme intermediate during the ligand exchange phase of folding .
	manualset3
157547	5	410282	7	NULL	NULL	0	NULL	aquo-heme intermediate	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The greater number of histidines and the greater strength of ligation are expected to slow conversion of the histidine-misligated forms to the obligatory aquo-heme intermediate during the ligand exchange phase of folding .
	manualset3
157548	6	410282	7	NULL	NULL	0	NULL	ligand exchange phase of folding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The greater number of histidines and the greater strength of ligation are expected to slow conversion of the histidine-misligated forms to the obligatory aquo-heme intermediate during the ligand exchange phase of folding .
	manualset3
157550	1	410283	7	NULL	NULL	0	NULL	greatest activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The greatest activity of the TREX1 protein was detected using a partial duplex DNA containing five mispaired nucleotides at the 3 ' terminus .
	manualset3
157551	2	410283	7	NULL	NULL	0	NULL	TREX1 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The greatest activity of the TREX1 protein was detected using a partial duplex DNA containing five mispaired nucleotides at the 3 ' terminus .
	manualset3
157552	3	410283	7	NULL	NULL	0	NULL	partial duplex DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The greatest activity of the TREX1 protein was detected using a partial duplex DNA containing five mispaired nucleotides at the 3 ' terminus .
	manualset3
157553	4	410283	7	NULL	NULL	0	NULL	five mispaired nucleotides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The greatest activity of the TREX1 protein was detected using a partial duplex DNA containing five mispaired nucleotides at the 3 ' terminus .
	manualset3
157554	5	410283	7	NULL	NULL	0	NULL	 3 ' terminus	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The greatest activity of the TREX1 protein was detected using a partial duplex DNA containing five mispaired nucleotides at the 3 ' terminus .
	manualset3
157555	1	410284	7	NULL	NULL	0	NULL	 greatest antiviral activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The greatest antiviral activity was shown by ara-AMP , and the least by ara-Hx .
	manualset3
157556	2	410284	7	NULL	NULL	0	NULL	ara-AMP	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The greatest antiviral activity was shown by ara-AMP , and the least by ara-Hx .
	manualset3
157557	3	410284	7	NULL	NULL	0	NULL	least	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The greatest antiviral activity was shown by ara-AMP , and the least by ara-Hx .
	manualset3
157558	4	410284	7	NULL	NULL	0	NULL	ara-Hx	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The greatest antiviral activity was shown by ara-AMP , and the least by ara-Hx .
	manualset3
157559	1	410285	7	NULL	NULL	NULL	NULL	mean percent  increase in ( 3H ) FLU binding	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The greatest mean percent increase in ( 3H ) FLU binding occurred in the medulla , including areas known to be important for cardiovascular control , breathing , motor tone and regulating levels of arousal .
	manualset3
157561	3	410285	7	NULL	NULL	0	NULL	medulla	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The greatest mean percent increase in ( 3H ) FLU binding occurred in the medulla , including areas known to be important for cardiovascular control , breathing , motor tone and regulating levels of arousal .
	manualset3
157562	5	410285	7	NULL	NULL	NULL	NULL	cardiovascular control	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The greatest mean percent increase in ( 3H ) FLU binding occurred in the medulla , including areas known to be important for cardiovascular control , breathing , motor tone and regulating levels of arousal .
	manualset3
157563	6	410285	7	NULL	NULL	NULL	NULL	breathing	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The greatest mean percent increase in ( 3H ) FLU binding occurred in the medulla , including areas known to be important for cardiovascular control , breathing , motor tone and regulating levels of arousal .
	manualset3
157564	7	410285	7	NULL	NULL	NULL	NULL	motor tone	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The greatest mean percent increase in ( 3H ) FLU binding occurred in the medulla , including areas known to be important for cardiovascular control , breathing , motor tone and regulating levels of arousal .
	manualset3
157565	8	410285	7	NULL	NULL	NULL	NULL	levels of arousal	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The greatest mean percent increase in ( 3H ) FLU binding occurred in the medulla , including areas known to be important for cardiovascular control , breathing , motor tone and regulating levels of arousal .
	manualset3
158510	4	410285	7	NULL	NULL	0	NULL	areas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The greatest mean percent increase in ( 3H ) FLU binding occurred in the medulla , including areas known to be important for cardiovascular control , breathing , motor tone and regulating levels of arousal .
	manualset3
157566	1	410286	7	NULL	NULL	0	NULL	greatest risk factors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The greatest risk factors for those over 69 years old were arterial hypertension , earlier episodes of TIA , diabetes , auricular fibrillation , congestive cardiac insufficiency , chronic bronchitis , myocardial infarction peripheral vascular-diseases , arteriosclerosis , heart disease with embolization and alcohol abuse .
	manualset3
157567	2	410286	7	NULL	NULL	0	NULL	69 years old	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The greatest risk factors for those over 69 years old were arterial hypertension , earlier episodes of TIA , diabetes , auricular fibrillation , congestive cardiac insufficiency , chronic bronchitis , myocardial infarction peripheral vascular-diseases , arteriosclerosis , heart disease with embolization and alcohol abuse .
	manualset3
157568	3	410286	7	NULL	NULL	0	NULL	arterial hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The greatest risk factors for those over 69 years old were arterial hypertension , earlier episodes of TIA , diabetes , auricular fibrillation , congestive cardiac insufficiency , chronic bronchitis , myocardial infarction peripheral vascular-diseases , arteriosclerosis , heart disease with embolization and alcohol abuse .
	manualset3
157569	4	410286	7	NULL	NULL	0	NULL	episodes of TIA	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The greatest risk factors for those over 69 years old were arterial hypertension , earlier episodes of TIA , diabetes , auricular fibrillation , congestive cardiac insufficiency , chronic bronchitis , myocardial infarction peripheral vascular-diseases , arteriosclerosis , heart disease with embolization and alcohol abuse .
	manualset3
157570	5	410286	7	NULL	NULL	0	NULL	 diabetes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The greatest risk factors for those over 69 years old were arterial hypertension , earlier episodes of TIA , diabetes , auricular fibrillation , congestive cardiac insufficiency , chronic bronchitis , myocardial infarction peripheral vascular-diseases , arteriosclerosis , heart disease with embolization and alcohol abuse .
	manualset3
157571	6	410286	7	NULL	NULL	0	NULL	auricular fibrillation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The greatest risk factors for those over 69 years old were arterial hypertension , earlier episodes of TIA , diabetes , auricular fibrillation , congestive cardiac insufficiency , chronic bronchitis , myocardial infarction peripheral vascular-diseases , arteriosclerosis , heart disease with embolization and alcohol abuse .
	manualset3
157572	7	410286	7	NULL	NULL	0	NULL	congestive cardiac insufficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The greatest risk factors for those over 69 years old were arterial hypertension , earlier episodes of TIA , diabetes , auricular fibrillation , congestive cardiac insufficiency , chronic bronchitis , myocardial infarction peripheral vascular-diseases , arteriosclerosis , heart disease with embolization and alcohol abuse .
	manualset3
157573	8	410286	7	NULL	NULL	NULL	NULL	chronic bronchitis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The greatest risk factors for those over 69 years old were arterial hypertension , earlier episodes of TIA , diabetes , auricular fibrillation , congestive cardiac insufficiency , chronic bronchitis , myocardial infarction peripheral vascular-diseases , arteriosclerosis , heart disease with embolization and alcohol abuse .
	manualset3
157574	9	410286	7	NULL	NULL	NULL	NULL	myocardial infarction peripheral vascular-diseases	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The greatest risk factors for those over 69 years old were arterial hypertension , earlier episodes of TIA , diabetes , auricular fibrillation , congestive cardiac insufficiency , chronic bronchitis , myocardial infarction peripheral vascular-diseases , arteriosclerosis , heart disease with embolization and alcohol abuse .
	manualset3
157575	10	410286	7	NULL	NULL	NULL	NULL	arteriosclerosis 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The greatest risk factors for those over 69 years old were arterial hypertension , earlier episodes of TIA , diabetes , auricular fibrillation , congestive cardiac insufficiency , chronic bronchitis , myocardial infarction peripheral vascular-diseases , arteriosclerosis , heart disease with embolization and alcohol abuse .
	manualset3
157576	11	410286	7	NULL	NULL	NULL	NULL	heart disease with embolization	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The greatest risk factors for those over 69 years old were arterial hypertension , earlier episodes of TIA , diabetes , auricular fibrillation , congestive cardiac insufficiency , chronic bronchitis , myocardial infarction peripheral vascular-diseases , arteriosclerosis , heart disease with embolization and alcohol abuse .
	manualset3
157577	12	410286	7	NULL	NULL	NULL	NULL	alcohol abuse	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The greatest risk factors for those over 69 years old were arterial hypertension , earlier episodes of TIA , diabetes , auricular fibrillation , congestive cardiac insufficiency , chronic bronchitis , myocardial infarction peripheral vascular-diseases , arteriosclerosis , heart disease with embolization and alcohol abuse .
	manualset3
157578	1	410287	7	NULL	NULL	0	NULL	 green tea component 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The green tea component epigallocatechin-3-gallate ( EGCG ) may be beneficial in autoimmune diseases ; however , the underlying mechanisms are not well understood .
	manualset3
157579	2	410287	7	NULL	NULL	0	NULL	epigallocatechin-3-gallate ( EGCG )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The green tea component epigallocatechin-3-gallate ( EGCG ) may be beneficial in autoimmune diseases ; however , the underlying mechanisms are not well understood .
	manualset3
157580	3	410287	7	NULL	NULL	0	NULL	autoimmune diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The green tea component epigallocatechin-3-gallate ( EGCG ) may be beneficial in autoimmune diseases ; however , the underlying mechanisms are not well understood .
	manualset3
157581	4	410287	7	NULL	NULL	0	NULL	mechanisms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The green tea component epigallocatechin-3-gallate ( EGCG ) may be beneficial in autoimmune diseases ; however , the underlying mechanisms are not well understood .
	manualset3
157582	1	410288	7	NULL	NULL	0	NULL	grid 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The grid was supported by a formvar film .
	manualset3
157583	2	410288	7	NULL	NULL	0	NULL	formvar film	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The grid was supported by a formvar film .
	manualset3
157584	1	410289	7	NULL	NULL	0	NULL	 ground reaction forces	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ground reaction forces of each leg reflect different roles , roughly corresponding to support , propulsion , and motion control as proposed by the hypothesis of functional asymmetry in human walking .
	manualset3
157585	2	410289	7	NULL	NULL	0	NULL	 leg 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The ground reaction forces of each leg reflect different roles , roughly corresponding to support , propulsion , and motion control as proposed by the hypothesis of functional asymmetry in human walking .
	manualset3
157586	3	410289	7	NULL	NULL	0	NULL	 roles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ground reaction forces of each leg reflect different roles , roughly corresponding to support , propulsion , and motion control as proposed by the hypothesis of functional asymmetry in human walking .
	manualset3
157587	4	410289	7	NULL	NULL	NULL	NULL	propulsion	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ground reaction forces of each leg reflect different roles , roughly corresponding to support , propulsion , and motion control as proposed by the hypothesis of functional asymmetry in human walking .
	manualset3
157588	5	410289	7	NULL	NULL	NULL	NULL	motion control	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ground reaction forces of each leg reflect different roles , roughly corresponding to support , propulsion , and motion control as proposed by the hypothesis of functional asymmetry in human walking .
	manualset3
157589	6	410289	7	NULL	NULL	NULL	NULL	hypothesis of functional asymmetry	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ground reaction forces of each leg reflect different roles , roughly corresponding to support , propulsion , and motion control as proposed by the hypothesis of functional asymmetry in human walking .
	manualset3
157590	7	410289	7	NULL	NULL	NULL	NULL	human walking	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ground reaction forces of each leg reflect different roles , roughly corresponding to support , propulsion , and motion control as proposed by the hypothesis of functional asymmetry in human walking .
	manualset3
158511	8	410289	7	NULL	NULL	0	NULL	support	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ground reaction forces of each leg reflect different roles , roughly corresponding to support , propulsion , and motion control as proposed by the hypothesis of functional asymmetry in human walking .
	manualset3
157591	1	410290	7	NULL	NULL	0	NULL	group A streptococcus ( GAS )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The group A streptococcus ( GAS ) , or Streptococcus pyogenes , is a strict human pathogen of medical significance , causing infections ranging from pharyngitis ( strep throat ) to necrotizing fasciitis ( flesh-eating disease ) .
	manualset3
157592	2	410290	7	NULL	NULL	0	NULL	Streptococcus pyogenes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The group A streptococcus ( GAS ) , or Streptococcus pyogenes , is a strict human pathogen of medical significance , causing infections ranging from pharyngitis ( strep throat ) to necrotizing fasciitis ( flesh-eating disease ) .
	manualset3
157593	3	410290	7	NULL	NULL	0	NULL	human pathogen	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The group A streptococcus ( GAS ) , or Streptococcus pyogenes , is a strict human pathogen of medical significance , causing infections ranging from pharyngitis ( strep throat ) to necrotizing fasciitis ( flesh-eating disease ) .
	manualset3
157594	5	410290	7	NULL	NULL	NULL	NULL	pharyngitis ( strep throat ) 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The group A streptococcus ( GAS ) , or Streptococcus pyogenes , is a strict human pathogen of medical significance , causing infections ranging from pharyngitis ( strep throat ) to necrotizing fasciitis ( flesh-eating disease ) .
	manualset3
157596	4	410290	7	NULL	NULL	NULL	NULL	infections	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The group A streptococcus ( GAS ) , or Streptococcus pyogenes , is a strict human pathogen of medical significance , causing infections ranging from pharyngitis ( strep throat ) to necrotizing fasciitis ( flesh-eating disease ) .
	manualset3
157597	6	410290	7	NULL	NULL	0	NULL	necrotizing fasciitis ( flesh-eating disease )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The group A streptococcus ( GAS ) , or Streptococcus pyogenes , is a strict human pathogen of medical significance , causing infections ranging from pharyngitis ( strep throat ) to necrotizing fasciitis ( flesh-eating disease ) .
	manualset3
159038	7	410290	7	NULL	NULL	0	NULL	medical significance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The group A streptococcus ( GAS ) , or Streptococcus pyogenes , is a strict human pathogen of medical significance , causing infections ranging from pharyngitis ( strep throat ) to necrotizing fasciitis ( flesh-eating disease ) .
	manualset3
157598	1	410291	7	NULL	NULL	0	NULL	interest	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The growing spark of interest in research concerning the molecular links between the nervous , endocrine and immune systems has caused an explosion of new knowledge concerning the fine mechanisms that orchestrate the integrated response to an immune challenge .
	manualset3
157599	2	410291	7	NULL	NULL	0	NULL	research 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The growing spark of interest in research concerning the molecular links between the nervous , endocrine and immune systems has caused an explosion of new knowledge concerning the fine mechanisms that orchestrate the integrated response to an immune challenge .
	manualset3
157600	3	410291	7	NULL	NULL	0	NULL	molecular links	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The growing spark of interest in research concerning the molecular links between the nervous , endocrine and immune systems has caused an explosion of new knowledge concerning the fine mechanisms that orchestrate the integrated response to an immune challenge .
	manualset3
157601	4	410291	7	NULL	NULL	0	NULL	nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The growing spark of interest in research concerning the molecular links between the nervous , endocrine and immune systems has caused an explosion of new knowledge concerning the fine mechanisms that orchestrate the integrated response to an immune challenge .
	manualset3
157602	5	410291	7	NULL	NULL	0	NULL	endocrine system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The growing spark of interest in research concerning the molecular links between the nervous , endocrine and immune systems has caused an explosion of new knowledge concerning the fine mechanisms that orchestrate the integrated response to an immune challenge .
	manualset3
157603	6	410291	7	NULL	NULL	0	NULL	immune systems	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The growing spark of interest in research concerning the molecular links between the nervous , endocrine and immune systems has caused an explosion of new knowledge concerning the fine mechanisms that orchestrate the integrated response to an immune challenge .
	manualset3
157604	7	410291	7	NULL	NULL	NULL	NULL	new knowledge	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The growing spark of interest in research concerning the molecular links between the nervous , endocrine and immune systems has caused an explosion of new knowledge concerning the fine mechanisms that orchestrate the integrated response to an immune challenge .
	manualset3
157605	8	410291	7	NULL	NULL	0	NULL	fine mechanisms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The growing spark of interest in research concerning the molecular links between the nervous , endocrine and immune systems has caused an explosion of new knowledge concerning the fine mechanisms that orchestrate the integrated response to an immune challenge .
	manualset3
157606	9	410291	7	NULL	NULL	NULL	NULL	response	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The growing spark of interest in research concerning the molecular links between the nervous , endocrine and immune systems has caused an explosion of new knowledge concerning the fine mechanisms that orchestrate the integrated response to an immune challenge .
	manualset3
157607	10	410291	7	NULL	NULL	0	NULL	immune challenge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The growing spark of interest in research concerning the molecular links between the nervous , endocrine and immune systems has caused an explosion of new knowledge concerning the fine mechanisms that orchestrate the integrated response to an immune challenge .
	manualset3
157608	1	410292	7	NULL	NULL	0	NULL	growth models	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The growth models accounted for up to 37.6 % of the initial error variance and provided evidence for two distinct , negatively correlated underlying trajectories of drinking patterns .
	manualset3
157609	2	410292	7	NULL	NULL	0	NULL	37.6 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The growth models accounted for up to 37.6 % of the initial error variance and provided evidence for two distinct , negatively correlated underlying trajectories of drinking patterns .
	manualset3
157610	3	410292	7	NULL	NULL	0	NULL	initial error variance	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The growth models accounted for up to 37.6 % of the initial error variance and provided evidence for two distinct , negatively correlated underlying trajectories of drinking patterns .
	manualset3
157611	4	410292	7	NULL	NULL	NULL	NULL	negatively correlated underlying trajectories	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The growth models accounted for up to 37.6 % of the initial error variance and provided evidence for two distinct , negatively correlated underlying trajectories of drinking patterns .
	manualset3
157612	5	410292	7	NULL	NULL	0	NULL	drinking patterns	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The growth models accounted for up to 37.6 % of the initial error variance and provided evidence for two distinct , negatively correlated underlying trajectories of drinking patterns .
	manualset3
159039	6	410292	7	NULL	NULL	0	NULL	evidence	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The growth models accounted for up to 37.6 % of the initial error variance and provided evidence for two distinct , negatively correlated underlying trajectories of drinking patterns .
	manualset3
157613	1	410293	7	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The growth of subcutaneously transplanted Lewis lung carcinoma in BDF1 mice was inhibited by an inorganic dye , Ruthenium Red .
	manualset3
157614	2	410293	7	NULL	NULL	NULL	NULL	subcutaneously transplanted Lewis lung carcinoma	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The growth of subcutaneously transplanted Lewis lung carcinoma in BDF1 mice was inhibited by an inorganic dye , Ruthenium Red .
	manualset3
157615	3	410293	7	NULL	NULL	0	NULL	BDF1 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The growth of subcutaneously transplanted Lewis lung carcinoma in BDF1 mice was inhibited by an inorganic dye , Ruthenium Red .
	manualset3
157616	4	410293	7	NULL	NULL	0	NULL	inorganic dye	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The growth of subcutaneously transplanted Lewis lung carcinoma in BDF1 mice was inhibited by an inorganic dye , Ruthenium Red .
	manualset3
157617	5	410293	7	NULL	NULL	0	NULL	Ruthenium Red	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The growth of subcutaneously transplanted Lewis lung carcinoma in BDF1 mice was inhibited by an inorganic dye , Ruthenium Red .
	manualset3
157618	1	410294	7	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The growth promoting effects of CT-1 therefore indicate that signaling pathways emanating from gp130 and LIFR are coupled to cardiomyocyte hypertrophy .
	manualset3
157619	2	410294	7	NULL	NULL	0	NULL	CT-1	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The growth promoting effects of CT-1 therefore indicate that signaling pathways emanating from gp130 and LIFR are coupled to cardiomyocyte hypertrophy .
	manualset3
157620	3	410294	7	NULL	NULL	0	NULL	signaling pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The growth promoting effects of CT-1 therefore indicate that signaling pathways emanating from gp130 and LIFR are coupled to cardiomyocyte hypertrophy .
	manualset3
157621	4	410294	7	NULL	NULL	0	NULL	gp130	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The growth promoting effects of CT-1 therefore indicate that signaling pathways emanating from gp130 and LIFR are coupled to cardiomyocyte hypertrophy .
	manualset3
157622	5	410294	7	NULL	NULL	0	NULL	LIFR	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The growth promoting effects of CT-1 therefore indicate that signaling pathways emanating from gp130 and LIFR are coupled to cardiomyocyte hypertrophy .
	manualset3
157623	6	410294	7	NULL	NULL	0	NULL	cardiomyocyte hypertrophy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The growth promoting effects of CT-1 therefore indicate that signaling pathways emanating from gp130 and LIFR are coupled to cardiomyocyte hypertrophy .
	manualset3
159040	7	410294	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The growth promoting effects of CT-1 therefore indicate that signaling pathways emanating from gp130 and LIFR are coupled to cardiomyocyte hypertrophy .
	manualset3
157624	1	410295	7	NULL	NULL	0	NULL	 Clinical  characteristics of non-malignant tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical and epidemiological characteristics of non-malignant tumors and the problem of their transformation into the malignant ones ( author 's transl ) ) .
	manualset3
157625	2	410295	7	NULL	NULL	0	NULL	epidemiological characteristics of non-malignant tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical and epidemiological characteristics of non-malignant tumors and the problem of their transformation into the malignant ones ( author 's transl ) ) .
	manualset3
157626	3	410295	7	NULL	NULL	0	NULL	problem	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical and epidemiological characteristics of non-malignant tumors and the problem of their transformation into the malignant ones ( author 's transl ) ) .
	manualset3
157627	4	410295	7	NULL	NULL	0	NULL	transformation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical and epidemiological characteristics of non-malignant tumors and the problem of their transformation into the malignant ones ( author 's transl ) ) .
	manualset3
157628	5	410295	7	NULL	NULL	0	NULL	malignant ones	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical and epidemiological characteristics of non-malignant tumors and the problem of their transformation into the malignant ones ( author 's transl ) ) .
	manualset3
157629	6	410295	7	NULL	NULL	0	NULL	author 's transl 	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical and epidemiological characteristics of non-malignant tumors and the problem of their transformation into the malignant ones ( author 's transl ) ) .
	manualset3
157630	1	410296	7	NULL	NULL	0	NULL	gut segments	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The gut segments which remove Cd from the hemolymph at the highest rate are the posterior midgut ( PMG ) and the ileum .
	manualset3
157631	2	410296	7	NULL	NULL	0	NULL	Cd 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The gut segments which remove Cd from the hemolymph at the highest rate are the posterior midgut ( PMG ) and the ileum .
	manualset3
157632	3	410296	7	NULL	NULL	0	NULL	hemolymph	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The gut segments which remove Cd from the hemolymph at the highest rate are the posterior midgut ( PMG ) and the ileum .
	manualset3
157633	4	410296	7	NULL	NULL	0	NULL	posterior midgut ( PMG )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The gut segments which remove Cd from the hemolymph at the highest rate are the posterior midgut ( PMG ) and the ileum .
	manualset3
157634	5	410296	7	NULL	NULL	0	NULL	ileum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The gut segments which remove Cd from the hemolymph at the highest rate are the posterior midgut ( PMG ) and the ileum .
	manualset3
159041	6	410296	7	NULL	NULL	0	NULL	highest rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The gut segments which remove Cd from the hemolymph at the highest rate are the posterior midgut ( PMG ) and the ileum .
	manualset3
157635	1	410297	7	NULL	NULL	NULL	NULL	hVPS34 product PI-3-K	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The hVPS34 product PI-3-K , according to the known data , is involved in the formation of internal vesicles of MVB .
	manualset3
157637	3	410297	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The hVPS34 product PI-3-K , according to the known data , is involved in the formation of internal vesicles of MVB .
	manualset3
157638	4	410297	7	NULL	NULL	0	NULL	formation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The hVPS34 product PI-3-K , according to the known data , is involved in the formation of internal vesicles of MVB .
	manualset3
157639	5	410297	7	NULL	NULL	0	NULL	internal vesicles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The hVPS34 product PI-3-K , according to the known data , is involved in the formation of internal vesicles of MVB .
	manualset3
157640	6	410297	7	NULL	NULL	0	NULL	MVB	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The hVPS34 product PI-3-K , according to the known data , is involved in the formation of internal vesicles of MVB .
	manualset3
157641	1	410298	7	NULL	NULL	0	NULL	half-life	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The half-life of 99mTc-albumin in the lung was 442 + / - 123 min during the control period , 363 + / - 52 min after detergent administration , and 134 + / - 18 min after oleic acid administration ( P less than 0.05 compared to control and P less than 0.01 compared to the period after detergent ) .
	manualset3
157642	2	410298	7	NULL	NULL	0	NULL	99mTc-albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The half-life of 99mTc-albumin in the lung was 442 + / - 123 min during the control period , 363 + / - 52 min after detergent administration , and 134 + / - 18 min after oleic acid administration ( P less than 0.05 compared to control and P less than 0.01 compared to the period after detergent ) .
	manualset3
157643	3	410298	7	NULL	NULL	0	NULL	lung	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The half-life of 99mTc-albumin in the lung was 442 + / - 123 min during the control period , 363 + / - 52 min after detergent administration , and 134 + / - 18 min after oleic acid administration ( P less than 0.05 compared to control and P less than 0.01 compared to the period after detergent ) .
	manualset3
157644	4	410298	7	NULL	NULL	NULL	NULL	 442 + / - 123 min	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The half-life of 99mTc-albumin in the lung was 442 + / - 123 min during the control period , 363 + / - 52 min after detergent administration , and 134 + / - 18 min after oleic acid administration ( P less than 0.05 compared to control and P less than 0.01 compared to the period after detergent ) .
	manualset3
157645	5	410298	7	NULL	NULL	0	NULL	control period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The half-life of 99mTc-albumin in the lung was 442 + / - 123 min during the control period , 363 + / - 52 min after detergent administration , and 134 + / - 18 min after oleic acid administration ( P less than 0.05 compared to control and P less than 0.01 compared to the period after detergent ) .
	manualset3
157646	6	410298	7	NULL	NULL	0	NULL	363 + / - 52 min	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The half-life of 99mTc-albumin in the lung was 442 + / - 123 min during the control period , 363 + / - 52 min after detergent administration , and 134 + / - 18 min after oleic acid administration ( P less than 0.05 compared to control and P less than 0.01 compared to the period after detergent ) .
	manualset3
157647	7	410298	7	NULL	NULL	NULL	NULL	 detergent administration	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The half-life of 99mTc-albumin in the lung was 442 + / - 123 min during the control period , 363 + / - 52 min after detergent administration , and 134 + / - 18 min after oleic acid administration ( P less than 0.05 compared to control and P less than 0.01 compared to the period after detergent ) .
	manualset3
157649	9	410298	7	NULL	NULL	0	NULL	134 + / - 18 min	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The half-life of 99mTc-albumin in the lung was 442 + / - 123 min during the control period , 363 + / - 52 min after detergent administration , and 134 + / - 18 min after oleic acid administration ( P less than 0.05 compared to control and P less than 0.01 compared to the period after detergent ) .
	manualset3
157650	10	410298	7	NULL	NULL	NULL	NULL	oleic acid administration	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The half-life of 99mTc-albumin in the lung was 442 + / - 123 min during the control period , 363 + / - 52 min after detergent administration , and 134 + / - 18 min after oleic acid administration ( P less than 0.05 compared to control and P less than 0.01 compared to the period after detergent ) .
	manualset3
157652	12	410298	7	NULL	NULL	0	NULL	P less than 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The half-life of 99mTc-albumin in the lung was 442 + / - 123 min during the control period , 363 + / - 52 min after detergent administration , and 134 + / - 18 min after oleic acid administration ( P less than 0.05 compared to control and P less than 0.01 compared to the period after detergent ) .
	manualset3
157653	13	410298	7	NULL	NULL	NULL	NULL	control	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The half-life of 99mTc-albumin in the lung was 442 + / - 123 min during the control period , 363 + / - 52 min after detergent administration , and 134 + / - 18 min after oleic acid administration ( P less than 0.05 compared to control and P less than 0.01 compared to the period after detergent ) .
	manualset3
157654	14	410298	7	NULL	NULL	0	NULL	P less than 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The half-life of 99mTc-albumin in the lung was 442 + / - 123 min during the control period , 363 + / - 52 min after detergent administration , and 134 + / - 18 min after oleic acid administration ( P less than 0.05 compared to control and P less than 0.01 compared to the period after detergent ) .
	manualset3
157655	15	410298	7	NULL	NULL	NULL	NULL	period after detergent	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The half-life of 99mTc-albumin in the lung was 442 + / - 123 min during the control period , 363 + / - 52 min after detergent administration , and 134 + / - 18 min after oleic acid administration ( P less than 0.05 compared to control and P less than 0.01 compared to the period after detergent ) .
	manualset3
157657	1	410299	7	NULL	NULL	0	NULL	half-life of the receptor	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The half-life of the receptor , as assessed by its disappearance after incubation with 18 microM cycloheximide was 8.4 hr in control cells and 10.3 hr and 5.0 hr in cells incubated with 0.25 and 4 mM butyrate , respectively .
	manualset3
157658	2	410299	7	NULL	NULL	0	NULL	incubation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The half-life of the receptor , as assessed by its disappearance after incubation with 18 microM cycloheximide was 8.4 hr in control cells and 10.3 hr and 5.0 hr in cells incubated with 0.25 and 4 mM butyrate , respectively .
	manualset3
157659	3	410299	7	NULL	NULL	0	NULL	18 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The half-life of the receptor , as assessed by its disappearance after incubation with 18 microM cycloheximide was 8.4 hr in control cells and 10.3 hr and 5.0 hr in cells incubated with 0.25 and 4 mM butyrate , respectively .
	manualset3
157660	4	410299	7	NULL	NULL	0	NULL	cycloheximide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The half-life of the receptor , as assessed by its disappearance after incubation with 18 microM cycloheximide was 8.4 hr in control cells and 10.3 hr and 5.0 hr in cells incubated with 0.25 and 4 mM butyrate , respectively .
	manualset3
157661	5	410299	7	NULL	NULL	0	NULL	8.4 hr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The half-life of the receptor , as assessed by its disappearance after incubation with 18 microM cycloheximide was 8.4 hr in control cells and 10.3 hr and 5.0 hr in cells incubated with 0.25 and 4 mM butyrate , respectively .
	manualset3
157662	6	410299	7	NULL	NULL	0	NULL	control cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The half-life of the receptor , as assessed by its disappearance after incubation with 18 microM cycloheximide was 8.4 hr in control cells and 10.3 hr and 5.0 hr in cells incubated with 0.25 and 4 mM butyrate , respectively .
	manualset3
157663	7	410299	7	NULL	NULL	0	NULL	10.3 hr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The half-life of the receptor , as assessed by its disappearance after incubation with 18 microM cycloheximide was 8.4 hr in control cells and 10.3 hr and 5.0 hr in cells incubated with 0.25 and 4 mM butyrate , respectively .
	manualset3
157664	8	410299	7	NULL	NULL	0	NULL	 5.0 hr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The half-life of the receptor , as assessed by its disappearance after incubation with 18 microM cycloheximide was 8.4 hr in control cells and 10.3 hr and 5.0 hr in cells incubated with 0.25 and 4 mM butyrate , respectively .
	manualset3
157665	9	410299	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The half-life of the receptor , as assessed by its disappearance after incubation with 18 microM cycloheximide was 8.4 hr in control cells and 10.3 hr and 5.0 hr in cells incubated with 0.25 and 4 mM butyrate , respectively .
	manualset3
157666	10	410299	7	NULL	NULL	0	NULL	0.25mM butyrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The half-life of the receptor , as assessed by its disappearance after incubation with 18 microM cycloheximide was 8.4 hr in control cells and 10.3 hr and 5.0 hr in cells incubated with 0.25 and 4 mM butyrate , respectively .
	manualset3
157667	11	410299	7	NULL	NULL	0	NULL	 4 mM butyrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The half-life of the receptor , as assessed by its disappearance after incubation with 18 microM cycloheximide was 8.4 hr in control cells and 10.3 hr and 5.0 hr in cells incubated with 0.25 and 4 mM butyrate , respectively .
	manualset3
159042	12	410299	7	NULL	NULL	0	NULL	disappearance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The half-life of the receptor , as assessed by its disappearance after incubation with 18 microM cycloheximide was 8.4 hr in control cells and 10.3 hr and 5.0 hr in cells incubated with 0.25 and 4 mM butyrate , respectively .
	manualset3
157668	1	410300	7	NULL	NULL	0	NULL	 handle region ( residues 84-99 )	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The handle region ( residues 84-99 ) in ribonuclease HI ( RNase HI ) from Escherichia coli , which is rich in basic amino acid residues , was altered by alanine-scanning mutagenesis .
	manualset3
157669	2	410300	7	NULL	NULL	0	NULL	ribonuclease HI ( RNase HI )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The handle region ( residues 84-99 ) in ribonuclease HI ( RNase HI ) from Escherichia coli , which is rich in basic amino acid residues , was altered by alanine-scanning mutagenesis .
	manualset3
157670	3	410300	7	NULL	NULL	0	NULL	Escherichia coli 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The handle region ( residues 84-99 ) in ribonuclease HI ( RNase HI ) from Escherichia coli , which is rich in basic amino acid residues , was altered by alanine-scanning mutagenesis .
	manualset3
157671	4	410300	7	NULL	NULL	0	NULL	basic amino acid residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The handle region ( residues 84-99 ) in ribonuclease HI ( RNase HI ) from Escherichia coli , which is rich in basic amino acid residues , was altered by alanine-scanning mutagenesis .
	manualset3
157672	5	410300	7	NULL	NULL	0	NULL	alanine-scanning mutagenesis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The handle region ( residues 84-99 ) in ribonuclease HI ( RNase HI ) from Escherichia coli , which is rich in basic amino acid residues , was altered by alanine-scanning mutagenesis .
	manualset3
157673	1	410301	7	NULL	NULL	0	NULL	haptens	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The haptens were linked to the carrier protein through hemisuccinate and hemisuccinylglycine bridges at the C-3 ' and C-3 '' positions in the digitoxose chain .
	manualset3
157674	2	410301	7	NULL	NULL	0	NULL	carrier protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The haptens were linked to the carrier protein through hemisuccinate and hemisuccinylglycine bridges at the C-3 ' and C-3 '' positions in the digitoxose chain .
	manualset3
157675	3	410301	7	NULL	NULL	0	NULL	hemisuccinate bridge	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The haptens were linked to the carrier protein through hemisuccinate and hemisuccinylglycine bridges at the C-3 ' and C-3 '' positions in the digitoxose chain .
	manualset3
157676	4	410301	7	NULL	NULL	0	NULL	hemisuccinylglycine bridge	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The haptens were linked to the carrier protein through hemisuccinate and hemisuccinylglycine bridges at the C-3 ' and C-3 '' positions in the digitoxose chain .
	manualset3
157677	5	410301	7	NULL	NULL	0	NULL	C-3 ' position	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The haptens were linked to the carrier protein through hemisuccinate and hemisuccinylglycine bridges at the C-3 ' and C-3 '' positions in the digitoxose chain .
	manualset3
157678	6	410301	7	NULL	NULL	0	NULL	C-3 '' position	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The haptens were linked to the carrier protein through hemisuccinate and hemisuccinylglycine bridges at the C-3 ' and C-3 '' positions in the digitoxose chain .
	manualset3
157679	7	410301	7	NULL	NULL	0	NULL	digitoxose chain	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The haptens were linked to the carrier protein through hemisuccinate and hemisuccinylglycine bridges at the C-3 ' and C-3 '' positions in the digitoxose chain .
	manualset3
157680	1	410302	7	NULL	NULL	0	NULL	hardness and Young 's modulus	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The hardness and Young 's modulus varied with location throughout the cross-sections from the occlusal surface to the dentin-enamel junction ( DEJ ) , from the buccal to lingual sides , and also from one tooth to another .
	manualset3
157681	2	410302	7	NULL	NULL	NULL	NULL	location	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The hardness and Young 's modulus varied with location throughout the cross-sections from the occlusal surface to the dentin-enamel junction ( DEJ ) , from the buccal to lingual sides , and also from one tooth to another .
	manualset3
157682	3	410302	7	NULL	NULL	0	NULL	cross-sections	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The hardness and Young 's modulus varied with location throughout the cross-sections from the occlusal surface to the dentin-enamel junction ( DEJ ) , from the buccal to lingual sides , and also from one tooth to another .
	manualset3
157683	4	410302	7	NULL	NULL	0	NULL	occlusal surface	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The hardness and Young 's modulus varied with location throughout the cross-sections from the occlusal surface to the dentin-enamel junction ( DEJ ) , from the buccal to lingual sides , and also from one tooth to another .
	manualset3
157684	5	410302	7	NULL	NULL	0	NULL	dentin-enamel junction ( DEJ )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The hardness and Young 's modulus varied with location throughout the cross-sections from the occlusal surface to the dentin-enamel junction ( DEJ ) , from the buccal to lingual sides , and also from one tooth to another .
	manualset3
157685	6	410302	7	NULL	NULL	NULL	NULL	buccal side	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The hardness and Young 's modulus varied with location throughout the cross-sections from the occlusal surface to the dentin-enamel junction ( DEJ ) , from the buccal to lingual sides , and also from one tooth to another .
	manualset3
157687	7	410302	7	NULL	NULL	0	NULL	lingual sides	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The hardness and Young 's modulus varied with location throughout the cross-sections from the occlusal surface to the dentin-enamel junction ( DEJ ) , from the buccal to lingual sides , and also from one tooth to another .
	manualset3
157688	8	410302	7	NULL	NULL	0	NULL	 one tooth	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The hardness and Young 's modulus varied with location throughout the cross-sections from the occlusal surface to the dentin-enamel junction ( DEJ ) , from the buccal to lingual sides , and also from one tooth to another .
	manualset3
157689	1	410303	7	NULL	NULL	NULL	NULL	harmonic distortion level	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The harmonic distortion level is generally obtained using the power spectrum of the audio signal from a loudspeaker , and a microphone is used to receive the audio signal .
	manualset3
157690	2	410303	7	NULL	NULL	0	NULL	power spectrum	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The harmonic distortion level is generally obtained using the power spectrum of the audio signal from a loudspeaker , and a microphone is used to receive the audio signal .
	manualset3
157691	3	410303	7	NULL	NULL	0	NULL	audio signal	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The harmonic distortion level is generally obtained using the power spectrum of the audio signal from a loudspeaker , and a microphone is used to receive the audio signal .
	manualset3
157692	4	410303	7	NULL	NULL	NULL	NULL	loudspeaker	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The harmonic distortion level is generally obtained using the power spectrum of the audio signal from a loudspeaker , and a microphone is used to receive the audio signal .
	manualset3
157693	5	410303	7	NULL	NULL	NULL	NULL	microphone	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The harmonic distortion level is generally obtained using the power spectrum of the audio signal from a loudspeaker , and a microphone is used to receive the audio signal .
	manualset3
157694	6	410303	7	NULL	NULL	0	NULL	audio signal	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The harmonic distortion level is generally obtained using the power spectrum of the audio signal from a loudspeaker , and a microphone is used to receive the audio signal .
	manualset3
157695	1	410304	7	NULL	NULL	0	NULL	harvested cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The harvested cells were analyzed by flow cytometry using monoclonal antibodies against leucocytes and macrophages .
	manualset3
157696	2	410304	7	NULL	NULL	0	NULL	flow cytometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The harvested cells were analyzed by flow cytometry using monoclonal antibodies against leucocytes and macrophages .
	manualset3
157697	3	410304	7	NULL	NULL	NULL	NULL	monoclonal antibodies 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The harvested cells were analyzed by flow cytometry using monoclonal antibodies against leucocytes and macrophages .
	manualset3
157698	4	410304	7	NULL	NULL	0	NULL	leucocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The harvested cells were analyzed by flow cytometry using monoclonal antibodies against leucocytes and macrophages .
	manualset3
157699	5	410304	7	NULL	NULL	0	NULL	macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The harvested cells were analyzed by flow cytometry using monoclonal antibodies against leucocytes and macrophages .
	manualset3
157700	1	410305	7	NULL	NULL	0	NULL	systematic search	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A systematic search for restriction fragment length polymorphisms ( RFLPs ) on the human Y chromosome was performed .
	manualset3
157701	2	410305	7	NULL	NULL	0	NULL	restriction fragment length polymorphisms ( RFLPs )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A systematic search for restriction fragment length polymorphisms ( RFLPs ) on the human Y chromosome was performed .
	manualset3
157702	3	410305	7	NULL	NULL	0	NULL	human Y chromosome	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	A systematic search for restriction fragment length polymorphisms ( RFLPs ) on the human Y chromosome was performed .
	manualset3
157703	1	410306	7	NULL	NULL	0	NULL	healing of wounds	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The healing of wounds by secondary intention is a simple method to close operative defects .
	manualset3
157704	2	410306	7	NULL	NULL	0	NULL	secondary intention	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The healing of wounds by secondary intention is a simple method to close operative defects .
	manualset3
157705	3	410306	7	NULL	NULL	0	NULL	simple method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The healing of wounds by secondary intention is a simple method to close operative defects .
	manualset3
157706	4	410306	7	NULL	NULL	0	NULL	operative defects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The healing of wounds by secondary intention is a simple method to close operative defects .
	manualset3
157707	1	410307	7	NULL	NULL	0	NULL	health care provider	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The health care provider can then anticipate problems , prepare the patient with accurate information , and institute interventions early to minimize symptoms .
	manualset3
157708	2	410307	7	NULL	NULL	0	NULL	problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The health care provider can then anticipate problems , prepare the patient with accurate information , and institute interventions early to minimize symptoms .
	manualset3
157709	3	410307	7	NULL	NULL	NULL	NULL	patient	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The health care provider can then anticipate problems , prepare the patient with accurate information , and institute interventions early to minimize symptoms .
	manualset3
157710	4	410307	7	NULL	NULL	0	NULL	accurate information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The health care provider can then anticipate problems , prepare the patient with accurate information , and institute interventions early to minimize symptoms .
	manualset3
157711	5	410307	7	NULL	NULL	NULL	NULL	institute interventions 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The health care provider can then anticipate problems , prepare the patient with accurate information , and institute interventions early to minimize symptoms .
	manualset3
157712	6	410307	7	NULL	NULL	0	NULL	symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The health care provider can then anticipate problems , prepare the patient with accurate information , and institute interventions early to minimize symptoms .
	manualset3
157713	1	410308	7	NULL	NULL	0	NULL	hearing loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The hearing loss is associated with inner ear abnormalities , ranging from an isolated enlarged vestibular aqueduct ( EVA ) to a typical coclear dysplasia .
	manualset3
157714	2	410308	7	NULL	NULL	0	NULL	 inner ear abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The hearing loss is associated with inner ear abnormalities , ranging from an isolated enlarged vestibular aqueduct ( EVA ) to a typical coclear dysplasia .
	manualset3
157715	3	410308	7	NULL	NULL	NULL	NULL	isolated enlarged vestibular aqueduct ( EVA )	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The hearing loss is associated with inner ear abnormalities , ranging from an isolated enlarged vestibular aqueduct ( EVA ) to a typical coclear dysplasia .
	manualset3
157716	4	410308	7	NULL	NULL	0	NULL	typical coclear dysplasia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The hearing loss is associated with inner ear abnormalities , ranging from an isolated enlarged vestibular aqueduct ( EVA ) to a typical coclear dysplasia .
	manualset3
157717	1	410309	7	NULL	NULL	0	NULL	 heart-to-mediastinum ( H/M ) MIBG uptake ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The heart-to-mediastinum ( H/M ) MIBG uptake ratio was evaluated , and the percent washout ratio of myocardial MIBG was obtained from these data .
	manualset3
157718	2	410309	7	NULL	NULL	0	NULL	percent washout ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The heart-to-mediastinum ( H/M ) MIBG uptake ratio was evaluated , and the percent washout ratio of myocardial MIBG was obtained from these data .
	manualset3
157719	3	410309	7	NULL	NULL	0	NULL	myocardial MIBG	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The heart-to-mediastinum ( H/M ) MIBG uptake ratio was evaluated , and the percent washout ratio of myocardial MIBG was obtained from these data .
	manualset3
157720	4	410309	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The heart-to-mediastinum ( H/M ) MIBG uptake ratio was evaluated , and the percent washout ratio of myocardial MIBG was obtained from these data .
	manualset3
157721	1	410310	7	NULL	NULL	0	NULL	heat shock protein gene ( HSP90 )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The heat shock protein gene ( HSP90 ) is induced at the early stage of differentiation and decreases to the basal level or under the basal level at the later stage .
	manualset3
157722	2	410310	7	NULL	NULL	0	NULL	early stage of differentiation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The heat shock protein gene ( HSP90 ) is induced at the early stage of differentiation and decreases to the basal level or under the basal level at the later stage .
	manualset3
157723	3	410310	7	NULL	NULL	0	NULL	basal level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The heat shock protein gene ( HSP90 ) is induced at the early stage of differentiation and decreases to the basal level or under the basal level at the later stage .
	manualset3
157724	4	410310	7	NULL	NULL	0	NULL	later stage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The heat shock protein gene ( HSP90 ) is induced at the early stage of differentiation and decreases to the basal level or under the basal level at the later stage .
	manualset3
157725	5	410310	7	NULL	NULL	0	NULL	basal level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The heat shock protein gene ( HSP90 ) is induced at the early stage of differentiation and decreases to the basal level or under the basal level at the later stage .
	manualset3
159043	6	410310	7	NULL	NULL	0	NULL	decreases	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The heat shock protein gene ( HSP90 ) is induced at the early stage of differentiation and decreases to the basal level or under the basal level at the later stage .
	manualset3
157726	1	410311	7	NULL	NULL	0	NULL	heavy incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The heavy incidence and severe or lethal damage caused by T. gondii infection clearly indicates the need for the development of a vaccine .
	manualset3
157727	2	410311	7	NULL	NULL	0	NULL	severe damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The heavy incidence and severe or lethal damage caused by T. gondii infection clearly indicates the need for the development of a vaccine .
	manualset3
157728	3	410311	7	NULL	NULL	0	NULL	lethal damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The heavy incidence and severe or lethal damage caused by T. gondii infection clearly indicates the need for the development of a vaccine .
	manualset3
157729	4	410311	7	NULL	NULL	0	NULL	T. gondii infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The heavy incidence and severe or lethal damage caused by T. gondii infection clearly indicates the need for the development of a vaccine .
	manualset3
157730	5	410311	7	NULL	NULL	0	NULL	 development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The heavy incidence and severe or lethal damage caused by T. gondii infection clearly indicates the need for the development of a vaccine .
	manualset3
157731	6	410311	7	NULL	NULL	0	NULL	vaccine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The heavy incidence and severe or lethal damage caused by T. gondii infection clearly indicates the need for the development of a vaccine .
	manualset3
157732	1	410312	7	NULL	NULL	NULL	NULL	helix unfolding	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The helix unfolding is found to proceed with a small positive heat-capacity increment , consistent with the solvation of some non-polar groups upon helix unfolding .
	manualset3
157733	2	410312	7	NULL	NULL	NULL	NULL	small positive heat-capacity increment	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The helix unfolding is found to proceed with a small positive heat-capacity increment , consistent with the solvation of some non-polar groups upon helix unfolding .
	manualset3
157734	3	410312	7	NULL	NULL	NULL	NULL	solvation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The helix unfolding is found to proceed with a small positive heat-capacity increment , consistent with the solvation of some non-polar groups upon helix unfolding .
	manualset3
157735	4	410312	7	NULL	NULL	0	NULL	non-polar groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The helix unfolding is found to proceed with a small positive heat-capacity increment , consistent with the solvation of some non-polar groups upon helix unfolding .
	manualset3
157736	5	410312	7	NULL	NULL	NULL	NULL	helix unfolding	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The helix unfolding is found to proceed with a small positive heat-capacity increment , consistent with the solvation of some non-polar groups upon helix unfolding .
	manualset3
157737	1	410313	7	NULL	NULL	0	NULL	hemiparesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The hemiparesis and speech disturbance improved almost completely after treatment , and her neck tremor has never occurred in one year follow-up .
	manualset3
157738	2	410313	7	NULL	NULL	0	NULL	speech disturbance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The hemiparesis and speech disturbance improved almost completely after treatment , and her neck tremor has never occurred in one year follow-up .
	manualset3
157739	3	410313	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The hemiparesis and speech disturbance improved almost completely after treatment , and her neck tremor has never occurred in one year follow-up .
	manualset3
157740	4	410313	7	NULL	NULL	0	NULL	neck tremor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The hemiparesis and speech disturbance improved almost completely after treatment , and her neck tremor has never occurred in one year follow-up .
	manualset3
157741	5	410313	7	NULL	NULL	0	NULL	one year	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The hemiparesis and speech disturbance improved almost completely after treatment , and her neck tremor has never occurred in one year follow-up .
	manualset3
157742	6	410313	7	NULL	NULL	0	NULL	follow-up 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The hemiparesis and speech disturbance improved almost completely after treatment , and her neck tremor has never occurred in one year follow-up .
	manualset3
157743	1	410314	7	NULL	NULL	0	NULL	hemoglobin calibration method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The hemoglobin calibration and quality assurance method proposed by Bull and colleagues is advocated as the presently most acceptable method .
	manualset3
157744	2	410314	7	NULL	NULL	0	NULL	quality assurance method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The hemoglobin calibration and quality assurance method proposed by Bull and colleagues is advocated as the presently most acceptable method .
	manualset3
157745	3	410314	7	NULL	NULL	0	NULL	Bull and colleagues	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	The hemoglobin calibration and quality assurance method proposed by Bull and colleagues is advocated as the presently most acceptable method .
	manualset3
157746	4	410314	7	NULL	NULL	0	NULL	method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The hemoglobin calibration and quality assurance method proposed by Bull and colleagues is advocated as the presently most acceptable method .
	manualset3
157747	1	410315	7	NULL	NULL	0	NULL	 hemostatic agent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The hemostatic agent used was one 500 mg capsule of tranxemic acid that was crushed and applied as a paste every 6 hourly .
	manualset3
157748	2	410315	7	NULL	NULL	0	NULL	500 mg capsule 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The hemostatic agent used was one 500 mg capsule of tranxemic acid that was crushed and applied as a paste every 6 hourly .
	manualset3
157749	3	410315	7	NULL	NULL	0	NULL	tranxemic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The hemostatic agent used was one 500 mg capsule of tranxemic acid that was crushed and applied as a paste every 6 hourly .
	manualset3
157750	4	410315	7	NULL	NULL	0	NULL	paste	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The hemostatic agent used was one 500 mg capsule of tranxemic acid that was crushed and applied as a paste every 6 hourly .
	manualset3
157751	5	410315	7	NULL	NULL	0	NULL	6	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The hemostatic agent used was one 500 mg capsule of tranxemic acid that was crushed and applied as a paste every 6 hourly .
	manualset3
157752	1	410316	7	NULL	NULL	0	NULL	hepatic microvascular	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The hepatic microvascular was generally intact with mild focal unfilled areas .
	manualset3
157753	2	410316	7	NULL	NULL	0	NULL	mild focal unfilled areas 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The hepatic microvascular was generally intact with mild focal unfilled areas .
	manualset3
157754	1	410317	7	NULL	NULL	0	NULL	heritability estimates	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The heritability estimates for lipoprotein ( a ) , apolipoprotein B , total cholesterol and HDL-C were 0.95 , 0.56 , 0.48 and 0.54 , respectively .
	manualset3
157755	2	410317	7	NULL	NULL	0	NULL	 lipoprotein ( a )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The heritability estimates for lipoprotein ( a ) , apolipoprotein B , total cholesterol and HDL-C were 0.95 , 0.56 , 0.48 and 0.54 , respectively .
	manualset3
157756	3	410317	7	NULL	NULL	0	NULL	apolipoprotein B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The heritability estimates for lipoprotein ( a ) , apolipoprotein B , total cholesterol and HDL-C were 0.95 , 0.56 , 0.48 and 0.54 , respectively .
	manualset3
157757	4	410317	7	NULL	NULL	0	NULL	 total cholesterol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The heritability estimates for lipoprotein ( a ) , apolipoprotein B , total cholesterol and HDL-C were 0.95 , 0.56 , 0.48 and 0.54 , respectively .
	manualset3
157758	5	410317	7	NULL	NULL	0	NULL	HDL-C	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The heritability estimates for lipoprotein ( a ) , apolipoprotein B , total cholesterol and HDL-C were 0.95 , 0.56 , 0.48 and 0.54 , respectively .
	manualset3
157759	6	410317	7	NULL	NULL	0	NULL	0.95	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The heritability estimates for lipoprotein ( a ) , apolipoprotein B , total cholesterol and HDL-C were 0.95 , 0.56 , 0.48 and 0.54 , respectively .
	manualset3
157760	7	410317	7	NULL	NULL	0	NULL	0.56	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The heritability estimates for lipoprotein ( a ) , apolipoprotein B , total cholesterol and HDL-C were 0.95 , 0.56 , 0.48 and 0.54 , respectively .
	manualset3
157761	8	410317	7	NULL	NULL	0	NULL	0.48	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The heritability estimates for lipoprotein ( a ) , apolipoprotein B , total cholesterol and HDL-C were 0.95 , 0.56 , 0.48 and 0.54 , respectively .
	manualset3
157762	9	410317	7	NULL	NULL	0	NULL	0.54	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The heritability estimates for lipoprotein ( a ) , apolipoprotein B , total cholesterol and HDL-C were 0.95 , 0.56 , 0.48 and 0.54 , respectively .
	manualset3
157763	1	410318	7	NULL	NULL	0	NULL	heterocyclic molecules in ( IV )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The heterocyclic molecules in ( IV ) are linked into chains of centrosymmetric rings by C-H ... O and C-H ... pi hydrogen bonds , again with the half-occupancy ethanol component pendent from the chain .
	manualset3
157764	2	410318	7	NULL	NULL	0	NULL	chains of centrosymmetric rings	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The heterocyclic molecules in ( IV ) are linked into chains of centrosymmetric rings by C-H ... O and C-H ... pi hydrogen bonds , again with the half-occupancy ethanol component pendent from the chain .
	manualset3
157765	3	410318	7	NULL	NULL	0	NULL	C-H ... O and C-H ... pi hydrogen bonds	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The heterocyclic molecules in ( IV ) are linked into chains of centrosymmetric rings by C-H ... O and C-H ... pi hydrogen bonds , again with the half-occupancy ethanol component pendent from the chain .
	manualset3
157766	4	410318	7	NULL	NULL	0	NULL	half-occupancy ethanol component pendent	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The heterocyclic molecules in ( IV ) are linked into chains of centrosymmetric rings by C-H ... O and C-H ... pi hydrogen bonds , again with the half-occupancy ethanol component pendent from the chain .
	manualset3
157767	5	410318	7	NULL	NULL	0	NULL	chain 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The heterocyclic molecules in ( IV ) are linked into chains of centrosymmetric rings by C-H ... O and C-H ... pi hydrogen bonds , again with the half-occupancy ethanol component pendent from the chain .
	manualset3
157768	1	410319	7	NULL	NULL	0	NULL	heterologous heterodimeric mutant gonadotropins 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The heterologous heterodimeric mutant and wild-type gonadotropins were equipotent in a competitive binding assay with ( 125I ) hCG .
	manualset3
157769	2	410319	7	NULL	NULL	0	NULL	heterologous heterodimeric  wild-type gonadotropins 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The heterologous heterodimeric mutant and wild-type gonadotropins were equipotent in a competitive binding assay with ( 125I ) hCG .
	manualset3
157770	3	410319	7	NULL	NULL	0	NULL	competitive binding assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The heterologous heterodimeric mutant and wild-type gonadotropins were equipotent in a competitive binding assay with ( 125I ) hCG .
	manualset3
157771	4	410319	7	NULL	NULL	0	NULL	( 125I ) hCG	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The heterologous heterodimeric mutant and wild-type gonadotropins were equipotent in a competitive binding assay with ( 125I ) hCG .
	manualset3
157772	5	410319	7	NULL	NULL	NULL	NULL	equipotent 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The heterologous heterodimeric mutant and wild-type gonadotropins were equipotent in a competitive binding assay with ( 125I ) hCG .
	manualset3
157773	1	410320	7	NULL	NULL	0	NULL	heterologous phase of desensitization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The heterologous phase of desensitization is slower , requiring 20-30 min of glucagon treatment to reach completion .
	manualset3
157774	2	410320	7	NULL	NULL	0	NULL	20-30 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The heterologous phase of desensitization is slower , requiring 20-30 min of glucagon treatment to reach completion .
	manualset3
157775	3	410320	7	NULL	NULL	0	NULL	 glucagon treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The heterologous phase of desensitization is slower , requiring 20-30 min of glucagon treatment to reach completion .
	manualset3
157776	4	410320	7	NULL	NULL	0	NULL	completion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The heterologous phase of desensitization is slower , requiring 20-30 min of glucagon treatment to reach completion .
	manualset3
157777	1	410321	7	NULL	NULL	0	NULL	hexane extract	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The hexane extract of the fruit of Schizandra chinensis ( Schisandraceae ) was found to show significant inhibition of the activity of acetylcholinesterase enzyme ( AChE ) .
	manualset3
157778	2	410321	7	NULL	NULL	0	NULL	fruit 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The hexane extract of the fruit of Schizandra chinensis ( Schisandraceae ) was found to show significant inhibition of the activity of acetylcholinesterase enzyme ( AChE ) .
	manualset3
157779	3	410321	7	NULL	NULL	0	NULL	 Schizandra chinensis ( Schisandraceae ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The hexane extract of the fruit of Schizandra chinensis ( Schisandraceae ) was found to show significant inhibition of the activity of acetylcholinesterase enzyme ( AChE ) .
	manualset3
157780	4	410321	7	NULL	NULL	0	NULL	inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The hexane extract of the fruit of Schizandra chinensis ( Schisandraceae ) was found to show significant inhibition of the activity of acetylcholinesterase enzyme ( AChE ) .
	manualset3
157781	5	410321	7	NULL	NULL	0	NULL	acetylcholinesterase enzyme ( AChE )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The hexane extract of the fruit of Schizandra chinensis ( Schisandraceae ) was found to show significant inhibition of the activity of acetylcholinesterase enzyme ( AChE ) .
	manualset3
159044	6	410321	7	NULL	NULL	0	NULL	activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The hexane extract of the fruit of Schizandra chinensis ( Schisandraceae ) was found to show significant inhibition of the activity of acetylcholinesterase enzyme ( AChE ) .
	manualset3
157782	1	410322	7	NULL	NULL	0	NULL	hierarchy	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The hierarchy is generated in real time in response to a user request .
	manualset3
157783	2	410322	7	NULL	NULL	0	NULL	real time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The hierarchy is generated in real time in response to a user request .
	manualset3
157784	3	410322	7	NULL	NULL	NULL	NULL	response	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The hierarchy is generated in real time in response to a user request .
	manualset3
157785	4	410322	7	NULL	NULL	NULL	NULL	user request	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The hierarchy is generated in real time in response to a user request .
	manualset3
157786	1	410323	7	NULL	NULL	0	NULL	high-fat diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The high-fat diet had 60 % of calories as fat and 20 % as carbohydrate .
	manualset3
157787	2	410323	7	NULL	NULL	0	NULL	60 % of calories	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The high-fat diet had 60 % of calories as fat and 20 % as carbohydrate .
	manualset3
157788	3	410323	7	NULL	NULL	NULL	NULL	fat	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The high-fat diet had 60 % of calories as fat and 20 % as carbohydrate .
	manualset3
157789	4	410323	7	NULL	NULL	NULL	NULL	20 % 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The high-fat diet had 60 % of calories as fat and 20 % as carbohydrate .
	manualset3
157790	5	410323	7	NULL	NULL	0	NULL	carbohydrate	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The high-fat diet had 60 % of calories as fat and 20 % as carbohydrate .
	manualset3
157791	1	410324	7	NULL	NULL	0	NULL	high-pressure phase 	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The high-pressure phase appears as a transparent crystalline mass. .
	manualset3
157792	2	410324	7	NULL	NULL	0	NULL	transparent crystalline mass	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The high-pressure phase appears as a transparent crystalline mass. .
	manualset3
157793	1	410325	7	NULL	NULL	0	NULL	high-resolution crystal structure	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The high-resolution crystal structure also reveals a hydrogen bond in both subunit types , but with subtly different geometry which may explain the very different behavior when this residue is mutated to glycine in alpha or beta globin .
	manualset3
157794	2	410325	7	NULL	NULL	0	NULL	hydrogen bond 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The high-resolution crystal structure also reveals a hydrogen bond in both subunit types , but with subtly different geometry which may explain the very different behavior when this residue is mutated to glycine in alpha or beta globin .
	manualset3
157795	3	410325	7	NULL	NULL	0	NULL	subunit types	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The high-resolution crystal structure also reveals a hydrogen bond in both subunit types , but with subtly different geometry which may explain the very different behavior when this residue is mutated to glycine in alpha or beta globin .
	manualset3
157796	4	410325	7	NULL	NULL	0	NULL	different geometry	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The high-resolution crystal structure also reveals a hydrogen bond in both subunit types , but with subtly different geometry which may explain the very different behavior when this residue is mutated to glycine in alpha or beta globin .
	manualset3
157797	5	410325	7	NULL	NULL	0	NULL	 behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The high-resolution crystal structure also reveals a hydrogen bond in both subunit types , but with subtly different geometry which may explain the very different behavior when this residue is mutated to glycine in alpha or beta globin .
	manualset3
157798	6	410325	7	NULL	NULL	0	NULL	residue 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The high-resolution crystal structure also reveals a hydrogen bond in both subunit types , but with subtly different geometry which may explain the very different behavior when this residue is mutated to glycine in alpha or beta globin .
	manualset3
157799	7	410325	7	NULL	NULL	0	NULL	glycine in alpha globin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The high-resolution crystal structure also reveals a hydrogen bond in both subunit types , but with subtly different geometry which may explain the very different behavior when this residue is mutated to glycine in alpha or beta globin .
	manualset3
157800	8	410325	7	NULL	NULL	0	NULL	glycine in beta globin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The high-resolution crystal structure also reveals a hydrogen bond in both subunit types , but with subtly different geometry which may explain the very different behavior when this residue is mutated to glycine in alpha or beta globin .
	manualset3
157801	1	410326	7	NULL	NULL	NULL	NULL	 purification	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The high degree of purification and low levels of contamination markers leave little doubt that the measured activities are intrinsic to myelin itself .
	manualset3
157802	2	410326	7	NULL	NULL	0	NULL	low levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The high degree of purification and low levels of contamination markers leave little doubt that the measured activities are intrinsic to myelin itself .
	manualset3
157803	3	410326	7	NULL	NULL	0	NULL	contamination markers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The high degree of purification and low levels of contamination markers leave little doubt that the measured activities are intrinsic to myelin itself .
	manualset3
157804	4	410326	7	NULL	NULL	0	NULL	myelin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The high degree of purification and low levels of contamination markers leave little doubt that the measured activities are intrinsic to myelin itself .
	manualset3
157805	5	410326	7	NULL	NULL	0	NULL	high degree	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The high degree of purification and low levels of contamination markers leave little doubt that the measured activities are intrinsic to myelin itself .
	manualset3
157806	1	410327	7	NULL	NULL	NULL	NULL	high efficacy	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The high efficacy of a complex therapy including beta-blockers and angioprotectors in concurrent IHD and diabetes is demonstrated .
	manualset3
157807	2	410327	7	NULL	NULL	0	NULL	complex therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The high efficacy of a complex therapy including beta-blockers and angioprotectors in concurrent IHD and diabetes is demonstrated .
	manualset3
157808	3	410327	7	NULL	NULL	NULL	NULL	 beta-blockers	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The high efficacy of a complex therapy including beta-blockers and angioprotectors in concurrent IHD and diabetes is demonstrated .
	manualset3
157809	4	410327	7	NULL	NULL	NULL	NULL	angioprotectors	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The high efficacy of a complex therapy including beta-blockers and angioprotectors in concurrent IHD and diabetes is demonstrated .
	manualset3
157810	5	410327	7	NULL	NULL	0	NULL	 IHD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The high efficacy of a complex therapy including beta-blockers and angioprotectors in concurrent IHD and diabetes is demonstrated .
	manualset3
157811	6	410327	7	NULL	NULL	0	NULL	diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The high efficacy of a complex therapy including beta-blockers and angioprotectors in concurrent IHD and diabetes is demonstrated .
	manualset3
157812	1	410328	7	NULL	NULL	0	NULL	high fiber diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The high fiber diet contained fruits and vegetables and the lower fiber diet contained fruit and vegetable juices .
	manualset3
157813	2	410328	7	NULL	NULL	0	NULL	fruits	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The high fiber diet contained fruits and vegetables and the lower fiber diet contained fruit and vegetable juices .
	manualset3
157814	3	410328	7	NULL	NULL	0	NULL	vegetables	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The high fiber diet contained fruits and vegetables and the lower fiber diet contained fruit and vegetable juices .
	manualset3
157815	4	410328	7	NULL	NULL	0	NULL	lower fiber diet 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The high fiber diet contained fruits and vegetables and the lower fiber diet contained fruit and vegetable juices .
	manualset3
157816	5	410328	7	NULL	NULL	0	NULL	fruit juice	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The high fiber diet contained fruits and vegetables and the lower fiber diet contained fruit and vegetable juices .
	manualset3
157817	6	410328	7	NULL	NULL	0	NULL	vegetable juice	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The high fiber diet contained fruits and vegetables and the lower fiber diet contained fruit and vegetable juices .
	manualset3
157818	1	410329	7	NULL	NULL	0	NULL	high incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The high incidence of Alzheimer 's disease associated with old age and the presence of its neuropathological signs in non-demented older individuals suggest that these two phenomena involve the same neurodegenerative processes and mechanisms and that Alzheimer 's disease is an extension of normal ageing .
	manualset3
157819	2	410329	7	NULL	NULL	0	NULL	Alzheimer 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The high incidence of Alzheimer 's disease associated with old age and the presence of its neuropathological signs in non-demented older individuals suggest that these two phenomena involve the same neurodegenerative processes and mechanisms and that Alzheimer 's disease is an extension of normal ageing .
	manualset3
157820	3	410329	7	NULL	NULL	NULL	NULL	old age	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The high incidence of Alzheimer 's disease associated with old age and the presence of its neuropathological signs in non-demented older individuals suggest that these two phenomena involve the same neurodegenerative processes and mechanisms and that Alzheimer 's disease is an extension of normal ageing .
	manualset3
157821	4	410329	7	NULL	NULL	NULL	NULL	neuropathological signs	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The high incidence of Alzheimer 's disease associated with old age and the presence of its neuropathological signs in non-demented older individuals suggest that these two phenomena involve the same neurodegenerative processes and mechanisms and that Alzheimer 's disease is an extension of normal ageing .
	manualset3
157822	5	410329	7	NULL	NULL	0	NULL	non-demented older individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The high incidence of Alzheimer 's disease associated with old age and the presence of its neuropathological signs in non-demented older individuals suggest that these two phenomena involve the same neurodegenerative processes and mechanisms and that Alzheimer 's disease is an extension of normal ageing .
	manualset3
157823	6	410329	7	NULL	NULL	NULL	NULL	phenomena	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The high incidence of Alzheimer 's disease associated with old age and the presence of its neuropathological signs in non-demented older individuals suggest that these two phenomena involve the same neurodegenerative processes and mechanisms and that Alzheimer 's disease is an extension of normal ageing .
	manualset3
157824	7	410329	7	NULL	NULL	0	NULL	neurodegenerative processes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The high incidence of Alzheimer 's disease associated with old age and the presence of its neuropathological signs in non-demented older individuals suggest that these two phenomena involve the same neurodegenerative processes and mechanisms and that Alzheimer 's disease is an extension of normal ageing .
	manualset3
157825	8	410329	7	NULL	NULL	0	NULL	mechanisms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The high incidence of Alzheimer 's disease associated with old age and the presence of its neuropathological signs in non-demented older individuals suggest that these two phenomena involve the same neurodegenerative processes and mechanisms and that Alzheimer 's disease is an extension of normal ageing .
	manualset3
157826	9	410329	7	NULL	NULL	0	NULL	Alzheimer 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The high incidence of Alzheimer 's disease associated with old age and the presence of its neuropathological signs in non-demented older individuals suggest that these two phenomena involve the same neurodegenerative processes and mechanisms and that Alzheimer 's disease is an extension of normal ageing .
	manualset3
157827	10	410329	7	NULL	NULL	0	NULL	normal ageing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The high incidence of Alzheimer 's disease associated with old age and the presence of its neuropathological signs in non-demented older individuals suggest that these two phenomena involve the same neurodegenerative processes and mechanisms and that Alzheimer 's disease is an extension of normal ageing .
	manualset3
157828	1	410330	7	NULL	NULL	0	NULL	high incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The high incidence of postoperative recurrence in Crohn 's disease mandates a strict follow-up ( clinical , laboratory and instrumental monitoring ) .
	manualset3
157829	2	410330	7	NULL	NULL	0	NULL	Crohn 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The high incidence of postoperative recurrence in Crohn 's disease mandates a strict follow-up ( clinical , laboratory and instrumental monitoring ) .
	manualset3
157830	3	410330	7	NULL	NULL	NULL	NULL	 follow-up 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The high incidence of postoperative recurrence in Crohn 's disease mandates a strict follow-up ( clinical , laboratory and instrumental monitoring ) .
	manualset3
158400	4	410330	7	NULL	NULL	0	NULL	 postoperative recurrence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The high incidence of postoperative recurrence in Crohn 's disease mandates a strict follow-up ( clinical , laboratory and instrumental monitoring ) .
	manualset3
159054	5	410330	7	NULL	NULL	0	NULL	clinical monitoring	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The high incidence of postoperative recurrence in Crohn 's disease mandates a strict follow-up ( clinical , laboratory and instrumental monitoring ) .
	manualset3
159055	6	410330	7	NULL	NULL	0	NULL	laboratory monitoring	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The high incidence of postoperative recurrence in Crohn 's disease mandates a strict follow-up ( clinical , laboratory and instrumental monitoring ) .
	manualset3
159056	7	410330	7	NULL	NULL	0	NULL	instrumental monitoring	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The high incidence of postoperative recurrence in Crohn 's disease mandates a strict follow-up ( clinical , laboratory and instrumental monitoring ) .
	manualset3
155488	1	410331	13	NULL	NULL	0	NULL	mass accuracy	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The high mass accuracy , resolution , capacity and scan rate of modern mass spectrometers have greatly facilitated this endeavor .
	manualset3
155489	2	410331	13	NULL	NULL	0	NULL	resolution	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The high mass accuracy , resolution , capacity and scan rate of modern mass spectrometers have greatly facilitated this endeavor .
	manualset3
155490	3	410331	13	NULL	NULL	0	NULL	capacity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The high mass accuracy , resolution , capacity and scan rate of modern mass spectrometers have greatly facilitated this endeavor .
	manualset3
155491	4	410331	13	NULL	NULL	0	NULL	scan rate 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The high mass accuracy , resolution , capacity and scan rate of modern mass spectrometers have greatly facilitated this endeavor .
	manualset3
155493	5	410331	13	NULL	NULL	0	NULL	modern mass spectrometers	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The high mass accuracy , resolution , capacity and scan rate of modern mass spectrometers have greatly facilitated this endeavor .
	manualset3
155495	6	410331	13	NULL	NULL	0	NULL	endeavor	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The high mass accuracy , resolution , capacity and scan rate of modern mass spectrometers have greatly facilitated this endeavor .
	manualset3
155497	1	410332	13	NULL	NULL	0	NULL	rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The high rate of CO2 assimilation ( 112-139 nmol / ( min mg protein ) ) and the cell yield ( 12 mg dry cells/mmol thiosulfate oxidized ) , 91-92 % of which was accounted for by CO2 carbon , were close to those typical of autotrophic bacteria .
	manualset3
155498	2	410332	13	NULL	NULL	0	NULL	CO2 assimilation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The high rate of CO2 assimilation ( 112-139 nmol / ( min mg protein ) ) and the cell yield ( 12 mg dry cells/mmol thiosulfate oxidized ) , 91-92 % of which was accounted for by CO2 carbon , were close to those typical of autotrophic bacteria .
	manualset3
155500	3	410332	13	NULL	NULL	0	NULL	112-139 nmol / ( min mg protein )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The high rate of CO2 assimilation ( 112-139 nmol / ( min mg protein ) ) and the cell yield ( 12 mg dry cells/mmol thiosulfate oxidized ) , 91-92 % of which was accounted for by CO2 carbon , were close to those typical of autotrophic bacteria .
	manualset3
155502	4	410332	13	NULL	NULL	0	NULL	cell yield	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The high rate of CO2 assimilation ( 112-139 nmol / ( min mg protein ) ) and the cell yield ( 12 mg dry cells/mmol thiosulfate oxidized ) , 91-92 % of which was accounted for by CO2 carbon , were close to those typical of autotrophic bacteria .
	manualset3
155503	5	410332	13	NULL	NULL	0	NULL	12 mg dry cells/mmol thiosulfate oxidized 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The high rate of CO2 assimilation ( 112-139 nmol / ( min mg protein ) ) and the cell yield ( 12 mg dry cells/mmol thiosulfate oxidized ) , 91-92 % of which was accounted for by CO2 carbon , were close to those typical of autotrophic bacteria .
	manualset3
155504	6	410332	13	NULL	NULL	0	NULL	91-92 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The high rate of CO2 assimilation ( 112-139 nmol / ( min mg protein ) ) and the cell yield ( 12 mg dry cells/mmol thiosulfate oxidized ) , 91-92 % of which was accounted for by CO2 carbon , were close to those typical of autotrophic bacteria .
	manualset3
155505	7	410332	13	NULL	NULL	0	NULL	CO2 carbon	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The high rate of CO2 assimilation ( 112-139 nmol / ( min mg protein ) ) and the cell yield ( 12 mg dry cells/mmol thiosulfate oxidized ) , 91-92 % of which was accounted for by CO2 carbon , were close to those typical of autotrophic bacteria .
	manualset3
155506	8	410332	13	NULL	NULL	0	NULL	 autotrophic bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The high rate of CO2 assimilation ( 112-139 nmol / ( min mg protein ) ) and the cell yield ( 12 mg dry cells/mmol thiosulfate oxidized ) , 91-92 % of which was accounted for by CO2 carbon , were close to those typical of autotrophic bacteria .
	manualset3
155511	1	410333	13	NULL	NULL	NULL	NULL	 t ( 1 ; 16 ) ( p22 ; p13 ) 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A t ( 1 ; 16 ) ( p22 ; p13 ) was found in the husband 's father and other relatives , and a t ( 1 ; 16 ) ( q24 ; q24 ) translocation in the proband 's family .
	manualset3
155513	2	410333	13	NULL	NULL	0	NULL	husband 's father	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A t ( 1 ; 16 ) ( p22 ; p13 ) was found in the husband 's father and other relatives , and a t ( 1 ; 16 ) ( q24 ; q24 ) translocation in the proband 's family .
	manualset3
155514	3	410333	13	NULL	NULL	0	NULL	 relatives 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A t ( 1 ; 16 ) ( p22 ; p13 ) was found in the husband 's father and other relatives , and a t ( 1 ; 16 ) ( q24 ; q24 ) translocation in the proband 's family .
	manualset3
155516	4	410333	13	NULL	NULL	0	NULL	t ( 1 ; 16 ) ( q24 ; q24 ) translocation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A t ( 1 ; 16 ) ( p22 ; p13 ) was found in the husband 's father and other relatives , and a t ( 1 ; 16 ) ( q24 ; q24 ) translocation in the proband 's family .
	manualset3
155517	5	410333	13	NULL	NULL	0	NULL	proband 's family	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A t ( 1 ; 16 ) ( p22 ; p13 ) was found in the husband 's father and other relatives , and a t ( 1 ; 16 ) ( q24 ; q24 ) translocation in the proband 's family .
	manualset3
155520	1	410334	13	NULL	NULL	0	NULL	total bilirubin	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The high total bilirubin and the low prothrombin time suggested serious liver dysfunction .
	manualset3
155522	2	410334	13	NULL	NULL	0	NULL	low prothrombin time 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The high total bilirubin and the low prothrombin time suggested serious liver dysfunction .
	manualset3
155524	3	410334	13	NULL	NULL	0	NULL	serious liver dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The high total bilirubin and the low prothrombin time suggested serious liver dysfunction .
	manualset3
155528	1	410335	13	NULL	NULL	0	NULL	concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The higher concentrations had reached statistical significance for all BCAAs by 6 hours , when leucine had risen by 83 % , isoleucine by 54 % , and valine by 47 % .
	manualset3
155530	2	410335	13	NULL	NULL	0	NULL	statistical significance	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The higher concentrations had reached statistical significance for all BCAAs by 6 hours , when leucine had risen by 83 % , isoleucine by 54 % , and valine by 47 % .
	manualset3
155531	3	410335	13	NULL	NULL	0	NULL	BCAAs	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The higher concentrations had reached statistical significance for all BCAAs by 6 hours , when leucine had risen by 83 % , isoleucine by 54 % , and valine by 47 % .
	manualset3
155533	4	410335	13	NULL	NULL	0	NULL	6 hours 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The higher concentrations had reached statistical significance for all BCAAs by 6 hours , when leucine had risen by 83 % , isoleucine by 54 % , and valine by 47 % .
	manualset3
155534	5	410335	13	NULL	NULL	0	NULL	leucine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The higher concentrations had reached statistical significance for all BCAAs by 6 hours , when leucine had risen by 83 % , isoleucine by 54 % , and valine by 47 % .
	manualset3
155535	6	410335	13	NULL	NULL	0	NULL	83 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The higher concentrations had reached statistical significance for all BCAAs by 6 hours , when leucine had risen by 83 % , isoleucine by 54 % , and valine by 47 % .
	manualset3
155537	7	410335	13	NULL	NULL	0	NULL	isoleucine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The higher concentrations had reached statistical significance for all BCAAs by 6 hours , when leucine had risen by 83 % , isoleucine by 54 % , and valine by 47 % .
	manualset3
155538	8	410335	13	NULL	NULL	0	NULL	54 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The higher concentrations had reached statistical significance for all BCAAs by 6 hours , when leucine had risen by 83 % , isoleucine by 54 % , and valine by 47 % .
	manualset3
155539	9	410335	13	NULL	NULL	0	NULL	valine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The higher concentrations had reached statistical significance for all BCAAs by 6 hours , when leucine had risen by 83 % , isoleucine by 54 % , and valine by 47 % .
	manualset3
155540	10	410335	13	NULL	NULL	0	NULL	47 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The higher concentrations had reached statistical significance for all BCAAs by 6 hours , when leucine had risen by 83 % , isoleucine by 54 % , and valine by 47 % .
	manualset3
155541	1	410336	13	NULL	NULL	0	NULL	doses	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest absorbed doses were generally the skin entrance doses .
	manualset3
155542	2	410336	13	NULL	NULL	0	NULL	skin entrance doses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest absorbed doses were generally the skin entrance doses .
	manualset3
155543	1	410337	13	NULL	NULL	0	NULL	accumulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest accumulation of endosulfan was found 24 hr after the start of the exposure to 1.5 ppm of the toxicant .
	manualset3
155544	2	410337	13	NULL	NULL	0	NULL	endosulfan	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest accumulation of endosulfan was found 24 hr after the start of the exposure to 1.5 ppm of the toxicant .
	manualset3
155545	3	410337	13	NULL	NULL	0	NULL	24 hr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest accumulation of endosulfan was found 24 hr after the start of the exposure to 1.5 ppm of the toxicant .
	manualset3
155546	4	410337	13	NULL	NULL	0	NULL	start	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest accumulation of endosulfan was found 24 hr after the start of the exposure to 1.5 ppm of the toxicant .
	manualset3
155547	5	410337	13	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest accumulation of endosulfan was found 24 hr after the start of the exposure to 1.5 ppm of the toxicant .
	manualset3
155548	6	410337	13	NULL	NULL	0	NULL	1.5 ppm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest accumulation of endosulfan was found 24 hr after the start of the exposure to 1.5 ppm of the toxicant .
	manualset3
155549	7	410337	13	NULL	NULL	0	NULL	toxicant 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest accumulation of endosulfan was found 24 hr after the start of the exposure to 1.5 ppm of the toxicant .
	manualset3
155550	1	410338	13	NULL	NULL	0	NULL	activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest activity towards bile acids is seen with lithocholic acid-24-methyl ester , and no activity is seen with lithocholic acid-3 alpha-sulfate or 5 beta - cholanic acid-3-one .
	manualset3
155551	2	410338	13	NULL	NULL	0	NULL	bile acids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest activity towards bile acids is seen with lithocholic acid-24-methyl ester , and no activity is seen with lithocholic acid-3 alpha-sulfate or 5 beta - cholanic acid-3-one .
	manualset3
155552	3	410338	13	NULL	NULL	0	NULL	 lithocholic acid-24-methyl ester	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest activity towards bile acids is seen with lithocholic acid-24-methyl ester , and no activity is seen with lithocholic acid-3 alpha-sulfate or 5 beta - cholanic acid-3-one .
	manualset3
155553	4	410338	13	NULL	NULL	0	NULL	activity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest activity towards bile acids is seen with lithocholic acid-24-methyl ester , and no activity is seen with lithocholic acid-3 alpha-sulfate or 5 beta - cholanic acid-3-one .
	manualset3
155554	5	410338	13	NULL	NULL	0	NULL	lithocholic acid-3 alpha-sulfate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest activity towards bile acids is seen with lithocholic acid-24-methyl ester , and no activity is seen with lithocholic acid-3 alpha-sulfate or 5 beta - cholanic acid-3-one .
	manualset3
155555	6	410338	13	NULL	NULL	0	NULL	5 beta - cholanic acid-3-one 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest activity towards bile acids is seen with lithocholic acid-24-methyl ester , and no activity is seen with lithocholic acid-3 alpha-sulfate or 5 beta - cholanic acid-3-one .
	manualset3
155556	1	410339	13	NULL	NULL	0	NULL	ammonium 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest ammonium adsorption capacity was observed for a zeolite particle size of 0.5 mm , which was 64 % and 31 % higher than that observed for particle sizes of 1.0 and 2.0 mm , respectively .
	manualset3
155557	2	410339	13	NULL	NULL	0	NULL	adsorption capacity 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest ammonium adsorption capacity was observed for a zeolite particle size of 0.5 mm , which was 64 % and 31 % higher than that observed for particle sizes of 1.0 and 2.0 mm , respectively .
	manualset3
155558	3	410339	13	NULL	NULL	0	NULL	 zeolite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest ammonium adsorption capacity was observed for a zeolite particle size of 0.5 mm , which was 64 % and 31 % higher than that observed for particle sizes of 1.0 and 2.0 mm , respectively .
	manualset3
155559	4	410339	13	NULL	NULL	0	NULL	particle size	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest ammonium adsorption capacity was observed for a zeolite particle size of 0.5 mm , which was 64 % and 31 % higher than that observed for particle sizes of 1.0 and 2.0 mm , respectively .
	manualset3
155560	5	410339	13	NULL	NULL	0	NULL	0.5 mm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest ammonium adsorption capacity was observed for a zeolite particle size of 0.5 mm , which was 64 % and 31 % higher than that observed for particle sizes of 1.0 and 2.0 mm , respectively .
	manualset3
155561	6	410339	13	NULL	NULL	0	NULL	64 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest ammonium adsorption capacity was observed for a zeolite particle size of 0.5 mm , which was 64 % and 31 % higher than that observed for particle sizes of 1.0 and 2.0 mm , respectively .
	manualset3
155562	7	410339	13	NULL	NULL	0	NULL	31 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest ammonium adsorption capacity was observed for a zeolite particle size of 0.5 mm , which was 64 % and 31 % higher than that observed for particle sizes of 1.0 and 2.0 mm , respectively .
	manualset3
155563	8	410339	13	NULL	NULL	0	NULL	particle sizes	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest ammonium adsorption capacity was observed for a zeolite particle size of 0.5 mm , which was 64 % and 31 % higher than that observed for particle sizes of 1.0 and 2.0 mm , respectively .
	manualset3
155564	9	410339	13	NULL	NULL	0	NULL	1.0 mm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest ammonium adsorption capacity was observed for a zeolite particle size of 0.5 mm , which was 64 % and 31 % higher than that observed for particle sizes of 1.0 and 2.0 mm , respectively .
	manualset3
155565	10	410339	13	NULL	NULL	0	NULL	2.0 mm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest ammonium adsorption capacity was observed for a zeolite particle size of 0.5 mm , which was 64 % and 31 % higher than that observed for particle sizes of 1.0 and 2.0 mm , respectively .
	manualset3
155566	1	410340	13	NULL	NULL	0	NULL	removal efficiencies	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest average removal efficiencies of 91 % for NH4-N , 59 % for PO4-P and 80 % for total chemical oxygen demand ( COD ) were achieved .
	manualset3
155567	2	410340	13	NULL	NULL	0	NULL	91 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest average removal efficiencies of 91 % for NH4-N , 59 % for PO4-P and 80 % for total chemical oxygen demand ( COD ) were achieved .
	manualset3
155568	3	410340	13	NULL	NULL	0	NULL	NH4-N	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest average removal efficiencies of 91 % for NH4-N , 59 % for PO4-P and 80 % for total chemical oxygen demand ( COD ) were achieved .
	manualset3
155569	4	410340	13	NULL	NULL	0	NULL	59 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest average removal efficiencies of 91 % for NH4-N , 59 % for PO4-P and 80 % for total chemical oxygen demand ( COD ) were achieved .
	manualset3
155570	5	410340	13	NULL	NULL	0	NULL	PO4-P 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest average removal efficiencies of 91 % for NH4-N , 59 % for PO4-P and 80 % for total chemical oxygen demand ( COD ) were achieved .
	manualset3
155571	6	410340	13	NULL	NULL	0	NULL	80 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest average removal efficiencies of 91 % for NH4-N , 59 % for PO4-P and 80 % for total chemical oxygen demand ( COD ) were achieved .
	manualset3
155572	7	410340	13	NULL	NULL	0	NULL	total chemical oxygen demand ( COD )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest average removal efficiencies of 91 % for NH4-N , 59 % for PO4-P and 80 % for total chemical oxygen demand ( COD ) were achieved .
	manualset3
155573	1	410341	13	NULL	NULL	0	NULL	concentration 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest concentration of proanthocyanidin in juice was found in Saskatoon berry ( 1363.34 mg/100 mL ) and the lowest value in strawberry ( 622.60 mg/100 mL ) .
	manualset3
155574	2	410341	13	NULL	NULL	0	NULL	proanthocyanidin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest concentration of proanthocyanidin in juice was found in Saskatoon berry ( 1363.34 mg/100 mL ) and the lowest value in strawberry ( 622.60 mg/100 mL ) .
	manualset3
155575	3	410341	13	NULL	NULL	0	NULL	juice 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest concentration of proanthocyanidin in juice was found in Saskatoon berry ( 1363.34 mg/100 mL ) and the lowest value in strawberry ( 622.60 mg/100 mL ) .
	manualset3
155576	4	410341	13	NULL	NULL	0	NULL	Saskatoon berry	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest concentration of proanthocyanidin in juice was found in Saskatoon berry ( 1363.34 mg/100 mL ) and the lowest value in strawberry ( 622.60 mg/100 mL ) .
	manualset3
155577	5	410341	13	NULL	NULL	0	NULL	1363.34 mg/100 mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest concentration of proanthocyanidin in juice was found in Saskatoon berry ( 1363.34 mg/100 mL ) and the lowest value in strawberry ( 622.60 mg/100 mL ) .
	manualset3
155578	6	410341	13	NULL	NULL	0	NULL	value	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest concentration of proanthocyanidin in juice was found in Saskatoon berry ( 1363.34 mg/100 mL ) and the lowest value in strawberry ( 622.60 mg/100 mL ) .
	manualset3
155579	7	410341	13	NULL	NULL	0	NULL	strawberry	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest concentration of proanthocyanidin in juice was found in Saskatoon berry ( 1363.34 mg/100 mL ) and the lowest value in strawberry ( 622.60 mg/100 mL ) .
	manualset3
155580	8	410341	13	NULL	NULL	0	NULL	622.60 mg/100 mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest concentration of proanthocyanidin in juice was found in Saskatoon berry ( 1363.34 mg/100 mL ) and the lowest value in strawberry ( 622.60 mg/100 mL ) .
	manualset3
155581	1	410342	13	NULL	NULL	0	NULL	dose	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest dose of NEA + EE was also maternally toxic , as two maternal deaths occurred at the end of the treatment period .
	manualset3
155582	2	410342	13	NULL	NULL	0	NULL	NEA + EE	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest dose of NEA + EE was also maternally toxic , as two maternal deaths occurred at the end of the treatment period .
	manualset3
155583	3	410342	13	NULL	NULL	0	NULL	two 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest dose of NEA + EE was also maternally toxic , as two maternal deaths occurred at the end of the treatment period .
	manualset3
155584	4	410342	13	NULL	NULL	0	NULL	maternal deaths	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest dose of NEA + EE was also maternally toxic , as two maternal deaths occurred at the end of the treatment period .
	manualset3
155585	5	410342	13	NULL	NULL	0	NULL	end 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest dose of NEA + EE was also maternally toxic , as two maternal deaths occurred at the end of the treatment period .
	manualset3
155586	6	410342	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest dose of NEA + EE was also maternally toxic , as two maternal deaths occurred at the end of the treatment period .
	manualset3
155587	7	410342	13	NULL	NULL	0	NULL	period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest dose of NEA + EE was also maternally toxic , as two maternal deaths occurred at the end of the treatment period .
	manualset3
155588	1	410343	13	NULL	NULL	0	NULL	temperatures	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest oceanic temperatures are found at hydrothermal vents , where the polychaete Paralvinella sulfincola lives on vent sulfides within steep and dynamic thermal gradients .
	manualset3
155589	2	410343	13	NULL	NULL	0	NULL	hydrothermal vents	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest oceanic temperatures are found at hydrothermal vents , where the polychaete Paralvinella sulfincola lives on vent sulfides within steep and dynamic thermal gradients .
	manualset3
155590	3	410343	13	NULL	NULL	0	NULL	polychaete Paralvinella sulfincola 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest oceanic temperatures are found at hydrothermal vents , where the polychaete Paralvinella sulfincola lives on vent sulfides within steep and dynamic thermal gradients .
	manualset3
155591	4	410343	13	NULL	NULL	0	NULL	lives	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest oceanic temperatures are found at hydrothermal vents , where the polychaete Paralvinella sulfincola lives on vent sulfides within steep and dynamic thermal gradients .
	manualset3
155592	5	410343	13	NULL	NULL	0	NULL	vent sulfides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest oceanic temperatures are found at hydrothermal vents , where the polychaete Paralvinella sulfincola lives on vent sulfides within steep and dynamic thermal gradients .
	manualset3
155593	6	410343	13	NULL	NULL	0	NULL	thermal gradients	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The highest oceanic temperatures are found at hydrothermal vents , where the polychaete Paralvinella sulfincola lives on vent sulfides within steep and dynamic thermal gradients .
	manualset3
155594	1	410344	13	NULL	NULL	0	NULL	volume fluctuations 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The highly damped volume fluctuations and their low temperature sensitivity , echo that PLFE liposomes are rigid and tightly packed .
	manualset3
155595	2	410344	13	NULL	NULL	0	NULL	temperature sensitivity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The highly damped volume fluctuations and their low temperature sensitivity , echo that PLFE liposomes are rigid and tightly packed .
	manualset3
155597	4	410344	13	NULL	NULL	0	NULL	PLFE liposomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The highly damped volume fluctuations and their low temperature sensitivity , echo that PLFE liposomes are rigid and tightly packed .
	manualset3
155598	1	410345	13	NULL	NULL	0	NULL	cis Golgi compartments	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The highly developed cis , medial and trans Golgi compartments reflect the biosynthetic and endocytotic activity of the gallbladder epithelium .
	manualset3
155599	2	410345	13	NULL	NULL	0	NULL	medial Golgi compartments	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The highly developed cis , medial and trans Golgi compartments reflect the biosynthetic and endocytotic activity of the gallbladder epithelium .
	manualset3
155600	3	410345	13	NULL	NULL	0	NULL	trans Golgi compartments 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The highly developed cis , medial and trans Golgi compartments reflect the biosynthetic and endocytotic activity of the gallbladder epithelium .
	manualset3
155601	4	410345	13	NULL	NULL	0	NULL	endocytotic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The highly developed cis , medial and trans Golgi compartments reflect the biosynthetic and endocytotic activity of the gallbladder epithelium .
	manualset3
155602	5	410345	13	NULL	NULL	0	NULL	gallbladder epithelium	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The highly developed cis , medial and trans Golgi compartments reflect the biosynthetic and endocytotic activity of the gallbladder epithelium .
	manualset3
157260	6	410345	13	NULL	NULL	0	NULL	biosynthetic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The highly developed cis , medial and trans Golgi compartments reflect the biosynthetic and endocytotic activity of the gallbladder epithelium .
	manualset3
155603	1	410346	13	NULL	NULL	0	NULL	tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The highly localized tissue effects of low energy femtosecond duration ( ultrashort ) laser pulses may be used to create three-dimensional intrastromal resections with micron precision and minimized collateral tissue damage .
	manualset3
155604	2	410346	13	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The highly localized tissue effects of low energy femtosecond duration ( ultrashort ) laser pulses may be used to create three-dimensional intrastromal resections with micron precision and minimized collateral tissue damage .
	manualset3
155605	3	410346	13	NULL	NULL	NULL	NULL	low energy femtosecond duration ( ultrashort ) laser pulses	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The highly localized tissue effects of low energy femtosecond duration ( ultrashort ) laser pulses may be used to create three-dimensional intrastromal resections with micron precision and minimized collateral tissue damage .
	manualset3
155607	4	410346	13	NULL	NULL	NULL	NULL	three-dimensional intrastromal resections	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The highly localized tissue effects of low energy femtosecond duration ( ultrashort ) laser pulses may be used to create three-dimensional intrastromal resections with micron precision and minimized collateral tissue damage .
	manualset3
155608	5	410346	13	NULL	NULL	NULL	NULL	micron precision	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The highly localized tissue effects of low energy femtosecond duration ( ultrashort ) laser pulses may be used to create three-dimensional intrastromal resections with micron precision and minimized collateral tissue damage .
	manualset3
155609	6	410346	13	NULL	NULL	NULL	NULL	tissue damage	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The highly localized tissue effects of low energy femtosecond duration ( ultrashort ) laser pulses may be used to create three-dimensional intrastromal resections with micron precision and minimized collateral tissue damage .
	manualset3
155610	1	410347	13	NULL	NULL	0	NULL	ribosome	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The highly stabilized ribosome display selection of metal binding peptide aptamers .
	manualset3
155611	2	410347	13	NULL	NULL	0	NULL	display	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The highly stabilized ribosome display selection of metal binding peptide aptamers .
	manualset3
155612	3	410347	13	NULL	NULL	0	NULL	selection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The highly stabilized ribosome display selection of metal binding peptide aptamers .
	manualset3
155613	4	410347	13	NULL	NULL	0	NULL	metal binding peptide aptamers 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The highly stabilized ribosome display selection of metal binding peptide aptamers .
	manualset3
155614	1	410348	13	NULL	NULL	0	NULL	 histamine level elevation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The histamine level elevation was greater in the portal venous blood than in the arterial blood .
	manualset3
155615	2	410348	13	NULL	NULL	0	NULL	portal venous blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The histamine level elevation was greater in the portal venous blood than in the arterial blood .
	manualset3
155616	3	410348	13	NULL	NULL	0	NULL	arterial blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The histamine level elevation was greater in the portal venous blood than in the arterial blood .
	manualset3
155617	1	410349	13	NULL	NULL	0	NULL	 histochemical evaluation	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The histochemical evaluation of alkaline phosphatase revealed an increased activity of the enzyme in the pial vessels of SHRs as compared with control rats with a similar localization of the enzyme activity .
	manualset3
155618	2	410349	13	NULL	NULL	0	NULL	alkaline phosphatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The histochemical evaluation of alkaline phosphatase revealed an increased activity of the enzyme in the pial vessels of SHRs as compared with control rats with a similar localization of the enzyme activity .
	manualset3
155619	3	410349	13	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The histochemical evaluation of alkaline phosphatase revealed an increased activity of the enzyme in the pial vessels of SHRs as compared with control rats with a similar localization of the enzyme activity .
	manualset3
155620	4	410349	13	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The histochemical evaluation of alkaline phosphatase revealed an increased activity of the enzyme in the pial vessels of SHRs as compared with control rats with a similar localization of the enzyme activity .
	manualset3
155621	5	410349	13	NULL	NULL	0	NULL	pial vessels 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The histochemical evaluation of alkaline phosphatase revealed an increased activity of the enzyme in the pial vessels of SHRs as compared with control rats with a similar localization of the enzyme activity .
	manualset3
155622	6	410349	13	NULL	NULL	0	NULL	 SHRs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The histochemical evaluation of alkaline phosphatase revealed an increased activity of the enzyme in the pial vessels of SHRs as compared with control rats with a similar localization of the enzyme activity .
	manualset3
155623	7	410349	13	NULL	NULL	0	NULL	control rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The histochemical evaluation of alkaline phosphatase revealed an increased activity of the enzyme in the pial vessels of SHRs as compared with control rats with a similar localization of the enzyme activity .
	manualset3
155624	8	410349	13	NULL	NULL	0	NULL	localization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The histochemical evaluation of alkaline phosphatase revealed an increased activity of the enzyme in the pial vessels of SHRs as compared with control rats with a similar localization of the enzyme activity .
	manualset3
155625	9	410349	13	NULL	NULL	0	NULL	enzyme activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The histochemical evaluation of alkaline phosphatase revealed an increased activity of the enzyme in the pial vessels of SHRs as compared with control rats with a similar localization of the enzyme activity .
	manualset3
155626	1	410350	13	NULL	NULL	0	NULL	histomorphological features	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The histomorphological features of hilar cholangiocarcinoma are identical with other extra - and intra-hepatic bile duct carcinomas .
	manualset3
155627	2	410350	13	NULL	NULL	0	NULL	hilar cholangiocarcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The histomorphological features of hilar cholangiocarcinoma are identical with other extra - and intra-hepatic bile duct carcinomas .
	manualset3
155628	3	410350	13	NULL	NULL	0	NULL	extra-hepatic bile duct carcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The histomorphological features of hilar cholangiocarcinoma are identical with other extra - and intra-hepatic bile duct carcinomas .
	manualset3
155629	4	410350	13	NULL	NULL	0	NULL	intra-hepatic bile duct carcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The histomorphological features of hilar cholangiocarcinoma are identical with other extra - and intra-hepatic bile duct carcinomas .
	manualset3
155630	1	410351	13	NULL	NULL	0	NULL	histopathologic features	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The histopathologic features of cytomegalovirus placentitis , an established cause of chronic villitis , are well documented .
	manualset3
155631	2	410351	13	NULL	NULL	0	NULL	cytomegalovirus placentitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The histopathologic features of cytomegalovirus placentitis , an established cause of chronic villitis , are well documented .
	manualset3
155632	3	410351	13	NULL	NULL	0	NULL	cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The histopathologic features of cytomegalovirus placentitis , an established cause of chronic villitis , are well documented .
	manualset3
155633	4	410351	13	NULL	NULL	0	NULL	chronic villitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The histopathologic features of cytomegalovirus placentitis , an established cause of chronic villitis , are well documented .
	manualset3
155634	1	410352	13	NULL	NULL	0	NULL	history 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The history of the service is presented and clinic staffing and operations are reviewed .
	manualset3
155635	2	410352	13	NULL	NULL	0	NULL	service 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The history of the service is presented and clinic staffing and operations are reviewed .
	manualset3
155636	3	410352	13	NULL	NULL	0	NULL	clinic	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The history of the service is presented and clinic staffing and operations are reviewed .
	manualset3
155637	4	410352	13	NULL	NULL	0	NULL	operations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The history of the service is presented and clinic staffing and operations are reviewed .
	manualset3
155638	1	410353	13	NULL	NULL	0	NULL	holoenzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The holoenzyme has a maximum of absorption at 362nm at pH7 .6 and 25 degrees C. 7 .
	manualset3
155639	2	410353	13	NULL	NULL	0	NULL	maximum	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The holoenzyme has a maximum of absorption at 362nm at pH7 .6 and 25 degrees C. 7 .
	manualset3
155640	3	410353	13	NULL	NULL	0	NULL	absorption	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The holoenzyme has a maximum of absorption at 362nm at pH7 .6 and 25 degrees C. 7 .
	manualset3
155641	4	410353	13	NULL	NULL	0	NULL	362nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The holoenzyme has a maximum of absorption at 362nm at pH7 .6 and 25 degrees C. 7 .
	manualset3
155642	5	410353	13	NULL	NULL	0	NULL	pH7 .6	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The holoenzyme has a maximum of absorption at 362nm at pH7 .6 and 25 degrees C. 7 .
	manualset3
155643	6	410353	13	NULL	NULL	0	NULL	25 degrees C. 7	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The holoenzyme has a maximum of absorption at 362nm at pH7 .6 and 25 degrees C. 7 .
	manualset3
155644	1	410354	13	NULL	NULL	0	NULL	homeotic genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The homeotic genes of the bithorax complex ( BX-C ) and the Antennapedia complex ( ANT-C ) of Drosophila appear to specify the developmental fate of segments or parts of segments of the fly .
	manualset3
155645	2	410354	13	NULL	NULL	0	NULL	bithorax complex ( BX-C ) 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The homeotic genes of the bithorax complex ( BX-C ) and the Antennapedia complex ( ANT-C ) of Drosophila appear to specify the developmental fate of segments or parts of segments of the fly .
	manualset3
155646	3	410354	13	NULL	NULL	0	NULL	Antennapedia complex ( ANT-C )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The homeotic genes of the bithorax complex ( BX-C ) and the Antennapedia complex ( ANT-C ) of Drosophila appear to specify the developmental fate of segments or parts of segments of the fly .
	manualset3
155647	4	410354	13	NULL	NULL	0	NULL	Drosophila 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The homeotic genes of the bithorax complex ( BX-C ) and the Antennapedia complex ( ANT-C ) of Drosophila appear to specify the developmental fate of segments or parts of segments of the fly .
	manualset3
155648	5	410354	13	NULL	NULL	0	NULL	developmental fate 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The homeotic genes of the bithorax complex ( BX-C ) and the Antennapedia complex ( ANT-C ) of Drosophila appear to specify the developmental fate of segments or parts of segments of the fly .
	manualset3
155649	6	410354	13	NULL	NULL	0	NULL	segments	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The homeotic genes of the bithorax complex ( BX-C ) and the Antennapedia complex ( ANT-C ) of Drosophila appear to specify the developmental fate of segments or parts of segments of the fly .
	manualset3
155650	7	410354	13	NULL	NULL	0	NULL	parts of segments 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The homeotic genes of the bithorax complex ( BX-C ) and the Antennapedia complex ( ANT-C ) of Drosophila appear to specify the developmental fate of segments or parts of segments of the fly .
	manualset3
155651	8	410354	13	NULL	NULL	0	NULL	fly	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The homeotic genes of the bithorax complex ( BX-C ) and the Antennapedia complex ( ANT-C ) of Drosophila appear to specify the developmental fate of segments or parts of segments of the fly .
	manualset3
155652	1	410355	13	NULL	NULL	0	NULL	hormone	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The hormone also increases the partially inhibited release of serotonin observed in platelets pretreated with the anti-GPIIb-IIIa antibody LJCP8 but does remove the total inhibition on the secretion caused by the anti-GPIb antibody LJIB1 .
	manualset3
155653	2	410355	13	NULL	NULL	0	NULL	release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The hormone also increases the partially inhibited release of serotonin observed in platelets pretreated with the anti-GPIIb-IIIa antibody LJCP8 but does remove the total inhibition on the secretion caused by the anti-GPIb antibody LJIB1 .
	manualset3
155654	3	410355	13	NULL	NULL	0	NULL	serotonin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The hormone also increases the partially inhibited release of serotonin observed in platelets pretreated with the anti-GPIIb-IIIa antibody LJCP8 but does remove the total inhibition on the secretion caused by the anti-GPIb antibody LJIB1 .
	manualset3
155655	4	410355	13	NULL	NULL	0	NULL	platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The hormone also increases the partially inhibited release of serotonin observed in platelets pretreated with the anti-GPIIb-IIIa antibody LJCP8 but does remove the total inhibition on the secretion caused by the anti-GPIb antibody LJIB1 .
	manualset3
155656	5	410355	13	NULL	NULL	0	NULL	anti-GPIIb-IIIa antibody LJCP8	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The hormone also increases the partially inhibited release of serotonin observed in platelets pretreated with the anti-GPIIb-IIIa antibody LJCP8 but does remove the total inhibition on the secretion caused by the anti-GPIb antibody LJIB1 .
	manualset3
155657	6	410355	13	NULL	NULL	0	NULL	inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The hormone also increases the partially inhibited release of serotonin observed in platelets pretreated with the anti-GPIIb-IIIa antibody LJCP8 but does remove the total inhibition on the secretion caused by the anti-GPIb antibody LJIB1 .
	manualset3
155658	7	410355	13	NULL	NULL	0	NULL	secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The hormone also increases the partially inhibited release of serotonin observed in platelets pretreated with the anti-GPIIb-IIIa antibody LJCP8 but does remove the total inhibition on the secretion caused by the anti-GPIb antibody LJIB1 .
	manualset3
155659	8	410355	13	NULL	NULL	0	NULL	anti-GPIb antibody LJIB1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The hormone also increases the partially inhibited release of serotonin observed in platelets pretreated with the anti-GPIIb-IIIa antibody LJCP8 but does remove the total inhibition on the secretion caused by the anti-GPIb antibody LJIB1 .
	manualset3
155660	1	410356	13	NULL	NULL	0	NULL	hospitalist movement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The hospitalist movement : ten issues to consider .
	manualset3
155661	2	410356	13	NULL	NULL	0	NULL	ten	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The hospitalist movement : ten issues to consider .
	manualset3
155662	3	410356	13	NULL	NULL	0	NULL	issues	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The hospitalist movement : ten issues to consider .
	manualset3
155663	1	410357	13	NULL	NULL	0	NULL	host factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The host factors smoking and atopy are not important confounding or effect-modifying factors in these relationships .
	manualset3
155664	2	410357	13	NULL	NULL	0	NULL	effect-modifying factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The host factors smoking and atopy are not important confounding or effect-modifying factors in these relationships .
	manualset3
155665	3	410357	13	NULL	NULL	0	NULL	relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The host factors smoking and atopy are not important confounding or effect-modifying factors in these relationships .
	manualset3
157261	4	410357	13	NULL	NULL	0	NULL	smoking	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The host factors smoking and atopy are not important confounding or effect-modifying factors in these relationships .
	manualset3
157262	5	410357	13	NULL	NULL	0	NULL	atopy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The host factors smoking and atopy are not important confounding or effect-modifying factors in these relationships .
	manualset3
155666	1	410358	13	NULL	NULL	0	NULL	host immune/inflammatory response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The host immune/inflammatory response following CNS infection by Klebsiella pneumoniae remains poorly understood .
	manualset3
155667	2	410358	13	NULL	NULL	0	NULL	CNS infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The host immune/inflammatory response following CNS infection by Klebsiella pneumoniae remains poorly understood .
	manualset3
155668	3	410358	13	NULL	NULL	0	NULL	 Klebsiella pneumoniae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The host immune/inflammatory response following CNS infection by Klebsiella pneumoniae remains poorly understood .
	manualset3
155669	1	410359	13	NULL	NULL	0	NULL	human legacy of cholera	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The human , societal , and scientific legacy of cholera .
	manualset3
155670	2	410359	13	NULL	NULL	0	NULL	societal legacy of cholera	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The human , societal , and scientific legacy of cholera .
	manualset3
155671	3	410359	13	NULL	NULL	0	NULL	scientific legacy of cholera	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The human , societal , and scientific legacy of cholera .
	manualset3
155672	1	410360	13	NULL	NULL	0	NULL	human P1 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The human P1 protein also shows significant similarity ( P less than 0.001 ) to a number of other bacterial and viral proteins including the pol polyprotein of human immunodeficiency viruses and the penicillin-binding protein of Neisseria gonorrhoeae .
	manualset3
155673	2	410360	13	NULL	NULL	0	NULL	similarity	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The human P1 protein also shows significant similarity ( P less than 0.001 ) to a number of other bacterial and viral proteins including the pol polyprotein of human immunodeficiency viruses and the penicillin-binding protein of Neisseria gonorrhoeae .
	manualset3
155674	3	410360	13	NULL	NULL	0	NULL	P less than 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The human P1 protein also shows significant similarity ( P less than 0.001 ) to a number of other bacterial and viral proteins including the pol polyprotein of human immunodeficiency viruses and the penicillin-binding protein of Neisseria gonorrhoeae .
	manualset3
155675	4	410360	13	NULL	NULL	0	NULL	 number	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The human P1 protein also shows significant similarity ( P less than 0.001 ) to a number of other bacterial and viral proteins including the pol polyprotein of human immunodeficiency viruses and the penicillin-binding protein of Neisseria gonorrhoeae .
	manualset3
155676	5	410360	13	NULL	NULL	0	NULL	bacterial proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The human P1 protein also shows significant similarity ( P less than 0.001 ) to a number of other bacterial and viral proteins including the pol polyprotein of human immunodeficiency viruses and the penicillin-binding protein of Neisseria gonorrhoeae .
	manualset3
155677	6	410360	13	NULL	NULL	0	NULL	viral proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The human P1 protein also shows significant similarity ( P less than 0.001 ) to a number of other bacterial and viral proteins including the pol polyprotein of human immunodeficiency viruses and the penicillin-binding protein of Neisseria gonorrhoeae .
	manualset3
155678	7	410360	13	NULL	NULL	0	NULL	pol polyprotein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The human P1 protein also shows significant similarity ( P less than 0.001 ) to a number of other bacterial and viral proteins including the pol polyprotein of human immunodeficiency viruses and the penicillin-binding protein of Neisseria gonorrhoeae .
	manualset3
155679	8	410360	13	NULL	NULL	0	NULL	human immunodeficiency viruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The human P1 protein also shows significant similarity ( P less than 0.001 ) to a number of other bacterial and viral proteins including the pol polyprotein of human immunodeficiency viruses and the penicillin-binding protein of Neisseria gonorrhoeae .
	manualset3
155680	9	410360	13	NULL	NULL	0	NULL	penicillin-binding protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The human P1 protein also shows significant similarity ( P less than 0.001 ) to a number of other bacterial and viral proteins including the pol polyprotein of human immunodeficiency viruses and the penicillin-binding protein of Neisseria gonorrhoeae .
	manualset3
155681	10	410360	13	NULL	NULL	0	NULL	Neisseria gonorrhoeae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The human P1 protein also shows significant similarity ( P less than 0.001 ) to a number of other bacterial and viral proteins including the pol polyprotein of human immunodeficiency viruses and the penicillin-binding protein of Neisseria gonorrhoeae .
	manualset3
155682	1	410361	13	NULL	NULL	0	NULL	human T-cell receptor Vbeta2 -encoding domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The human T-cell receptor Vbeta2 - , D - and J-encoding domains were PCR-amplified from MOLT-4 total cDNA and subcloned in Escherichia coli .
	manualset3
155683	2	410361	13	NULL	NULL	0	NULL	human T-cell receptor D -encoding domains 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The human T-cell receptor Vbeta2 - , D - and J-encoding domains were PCR-amplified from MOLT-4 total cDNA and subcloned in Escherichia coli .
	manualset3
155684	3	410361	13	NULL	NULL	0	NULL	human T-cell receptor J-encoding domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The human T-cell receptor Vbeta2 - , D - and J-encoding domains were PCR-amplified from MOLT-4 total cDNA and subcloned in Escherichia coli .
	manualset3
155685	4	410361	13	NULL	NULL	0	NULL	MOLT-4 total cDNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The human T-cell receptor Vbeta2 - , D - and J-encoding domains were PCR-amplified from MOLT-4 total cDNA and subcloned in Escherichia coli .
	manualset3
155686	5	410361	13	NULL	NULL	0	NULL	Escherichia coli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The human T-cell receptor Vbeta2 - , D - and J-encoding domains were PCR-amplified from MOLT-4 total cDNA and subcloned in Escherichia coli .
	manualset3
155687	1	410362	13	NULL	NULL	0	NULL	human brain 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The human brain , which is a structurally and dynamically complex device , not only perceives but also creates new reality : it is a hermeneutic device .
	manualset3
155688	2	410362	13	NULL	NULL	0	NULL	device	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The human brain , which is a structurally and dynamically complex device , not only perceives but also creates new reality : it is a hermeneutic device .
	manualset3
155689	3	410362	13	NULL	NULL	0	NULL	reality	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The human brain , which is a structurally and dynamically complex device , not only perceives but also creates new reality : it is a hermeneutic device .
	manualset3
155690	4	410362	13	NULL	NULL	0	NULL	hermeneutic device	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The human brain , which is a structurally and dynamically complex device , not only perceives but also creates new reality : it is a hermeneutic device .
	manualset3
155691	1	410363	13	NULL	NULL	0	NULL	human embryo	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The human embryo : a scientist 's point of view .
	manualset3
155692	2	410363	13	NULL	NULL	0	NULL	scientist 's	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The human embryo : a scientist 's point of view .
	manualset3
155693	3	410363	13	NULL	NULL	0	NULL	point of view	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The human embryo : a scientist 's point of view .
	manualset3
155694	1	410364	13	NULL	NULL	0	NULL	human gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The human gene for slow-twitch skeletal muscle troponin I ( TNNI1 ) has previously been mapped to 1q12 -- ) qter using somatic cell hybrids .
	manualset3
155695	2	410364	13	NULL	NULL	0	NULL	slow-twitch skeletal muscle troponin I ( TNNI1 ) 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The human gene for slow-twitch skeletal muscle troponin I ( TNNI1 ) has previously been mapped to 1q12 -- ) qter using somatic cell hybrids .
	manualset3
155696	3	410364	13	NULL	NULL	0	NULL	1q12 -- ) qter 	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The human gene for slow-twitch skeletal muscle troponin I ( TNNI1 ) has previously been mapped to 1q12 -- ) qter using somatic cell hybrids .
	manualset3
155697	4	410364	13	NULL	NULL	0	NULL	somatic cell hybrids	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The human gene for slow-twitch skeletal muscle troponin I ( TNNI1 ) has previously been mapped to 1q12 -- ) qter using somatic cell hybrids .
	manualset3
155698	1	410365	13	NULL	NULL	0	NULL	 human lexinome	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The human lexinome : genes of language and reading .
	manualset3
155699	2	410365	13	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The human lexinome : genes of language and reading .
	manualset3
155700	3	410365	13	NULL	NULL	0	NULL	language 	Language												NULL		0	NULL	NULL	NULL	NULL	NULL	The human lexinome : genes of language and reading .
	manualset3
155701	4	410365	13	NULL	NULL	0	NULL	reading	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The human lexinome : genes of language and reading .
	manualset3
155714	1	410366	13	NULL	NULL	NULL	NULL	human species	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The human species is exerting its influence through rapid human population growth ( projected to soar from 5.3 billion in 1990 to 10-12 billion a century from now ) , through escalating resource demand , ( especially in the wealthier countries with threatened changes in global climate and sea level ) , and through severe pressure of poverty in less developed countries which result in habitat transformations and losses of biological diversity .
	manualset3
155715	2	410366	13	NULL	NULL	0	NULL	influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The human species is exerting its influence through rapid human population growth ( projected to soar from 5.3 billion in 1990 to 10-12 billion a century from now ) , through escalating resource demand , ( especially in the wealthier countries with threatened changes in global climate and sea level ) , and through severe pressure of poverty in less developed countries which result in habitat transformations and losses of biological diversity .
	manualset3
155716	3	410366	13	NULL	NULL	0	NULL	human population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The human species is exerting its influence through rapid human population growth ( projected to soar from 5.3 billion in 1990 to 10-12 billion a century from now ) , through escalating resource demand , ( especially in the wealthier countries with threatened changes in global climate and sea level ) , and through severe pressure of poverty in less developed countries which result in habitat transformations and losses of biological diversity .
	manualset3
155717	4	410366	13	NULL	NULL	0	NULL	growth 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The human species is exerting its influence through rapid human population growth ( projected to soar from 5.3 billion in 1990 to 10-12 billion a century from now ) , through escalating resource demand , ( especially in the wealthier countries with threatened changes in global climate and sea level ) , and through severe pressure of poverty in less developed countries which result in habitat transformations and losses of biological diversity .
	manualset3
155718	5	410366	13	NULL	NULL	0	NULL	5.3 billion	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The human species is exerting its influence through rapid human population growth ( projected to soar from 5.3 billion in 1990 to 10-12 billion a century from now ) , through escalating resource demand , ( especially in the wealthier countries with threatened changes in global climate and sea level ) , and through severe pressure of poverty in less developed countries which result in habitat transformations and losses of biological diversity .
	manualset3
155719	6	410366	13	NULL	NULL	0	NULL	1990 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The human species is exerting its influence through rapid human population growth ( projected to soar from 5.3 billion in 1990 to 10-12 billion a century from now ) , through escalating resource demand , ( especially in the wealthier countries with threatened changes in global climate and sea level ) , and through severe pressure of poverty in less developed countries which result in habitat transformations and losses of biological diversity .
	manualset3
155720	7	410366	13	NULL	NULL	0	NULL	10-12 billion	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The human species is exerting its influence through rapid human population growth ( projected to soar from 5.3 billion in 1990 to 10-12 billion a century from now ) , through escalating resource demand , ( especially in the wealthier countries with threatened changes in global climate and sea level ) , and through severe pressure of poverty in less developed countries which result in habitat transformations and losses of biological diversity .
	manualset3
155721	8	410366	13	NULL	NULL	0	NULL	century	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The human species is exerting its influence through rapid human population growth ( projected to soar from 5.3 billion in 1990 to 10-12 billion a century from now ) , through escalating resource demand , ( especially in the wealthier countries with threatened changes in global climate and sea level ) , and through severe pressure of poverty in less developed countries which result in habitat transformations and losses of biological diversity .
	manualset3
155722	9	410366	13	NULL	NULL	0	NULL	resource	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The human species is exerting its influence through rapid human population growth ( projected to soar from 5.3 billion in 1990 to 10-12 billion a century from now ) , through escalating resource demand , ( especially in the wealthier countries with threatened changes in global climate and sea level ) , and through severe pressure of poverty in less developed countries which result in habitat transformations and losses of biological diversity .
	manualset3
155723	10	410366	13	NULL	NULL	0	NULL	wealthier countries	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The human species is exerting its influence through rapid human population growth ( projected to soar from 5.3 billion in 1990 to 10-12 billion a century from now ) , through escalating resource demand , ( especially in the wealthier countries with threatened changes in global climate and sea level ) , and through severe pressure of poverty in less developed countries which result in habitat transformations and losses of biological diversity .
	manualset3
155724	11	410366	13	NULL	NULL	0	NULL	global climate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The human species is exerting its influence through rapid human population growth ( projected to soar from 5.3 billion in 1990 to 10-12 billion a century from now ) , through escalating resource demand , ( especially in the wealthier countries with threatened changes in global climate and sea level ) , and through severe pressure of poverty in less developed countries which result in habitat transformations and losses of biological diversity .
	manualset3
155725	12	410366	13	NULL	NULL	0	NULL	sea level	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The human species is exerting its influence through rapid human population growth ( projected to soar from 5.3 billion in 1990 to 10-12 billion a century from now ) , through escalating resource demand , ( especially in the wealthier countries with threatened changes in global climate and sea level ) , and through severe pressure of poverty in less developed countries which result in habitat transformations and losses of biological diversity .
	manualset3
155726	13	410366	13	NULL	NULL	0	NULL	severe pressure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The human species is exerting its influence through rapid human population growth ( projected to soar from 5.3 billion in 1990 to 10-12 billion a century from now ) , through escalating resource demand , ( especially in the wealthier countries with threatened changes in global climate and sea level ) , and through severe pressure of poverty in less developed countries which result in habitat transformations and losses of biological diversity .
	manualset3
155727	14	410366	13	NULL	NULL	0	NULL	poverty 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The human species is exerting its influence through rapid human population growth ( projected to soar from 5.3 billion in 1990 to 10-12 billion a century from now ) , through escalating resource demand , ( especially in the wealthier countries with threatened changes in global climate and sea level ) , and through severe pressure of poverty in less developed countries which result in habitat transformations and losses of biological diversity .
	manualset3
155728	15	410366	13	NULL	NULL	0	NULL	countries	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The human species is exerting its influence through rapid human population growth ( projected to soar from 5.3 billion in 1990 to 10-12 billion a century from now ) , through escalating resource demand , ( especially in the wealthier countries with threatened changes in global climate and sea level ) , and through severe pressure of poverty in less developed countries which result in habitat transformations and losses of biological diversity .
	manualset3
155729	16	410366	13	NULL	NULL	0	NULL	result	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The human species is exerting its influence through rapid human population growth ( projected to soar from 5.3 billion in 1990 to 10-12 billion a century from now ) , through escalating resource demand , ( especially in the wealthier countries with threatened changes in global climate and sea level ) , and through severe pressure of poverty in less developed countries which result in habitat transformations and losses of biological diversity .
	manualset3
155730	17	410366	13	NULL	NULL	0	NULL	habitat transformations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The human species is exerting its influence through rapid human population growth ( projected to soar from 5.3 billion in 1990 to 10-12 billion a century from now ) , through escalating resource demand , ( especially in the wealthier countries with threatened changes in global climate and sea level ) , and through severe pressure of poverty in less developed countries which result in habitat transformations and losses of biological diversity .
	manualset3
155731	18	410366	13	NULL	NULL	0	NULL	losses	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The human species is exerting its influence through rapid human population growth ( projected to soar from 5.3 billion in 1990 to 10-12 billion a century from now ) , through escalating resource demand , ( especially in the wealthier countries with threatened changes in global climate and sea level ) , and through severe pressure of poverty in less developed countries which result in habitat transformations and losses of biological diversity .
	manualset3
155732	19	410366	13	NULL	NULL	0	NULL	biological diversity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The human species is exerting its influence through rapid human population growth ( projected to soar from 5.3 billion in 1990 to 10-12 billion a century from now ) , through escalating resource demand , ( especially in the wealthier countries with threatened changes in global climate and sea level ) , and through severe pressure of poverty in less developed countries which result in habitat transformations and losses of biological diversity .
	manualset3
157263	20	410366	13	NULL	NULL	0	NULL	changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The human species is exerting its influence through rapid human population growth ( projected to soar from 5.3 billion in 1990 to 10-12 billion a century from now ) , through escalating resource demand , ( especially in the wealthier countries with threatened changes in global climate and sea level ) , and through severe pressure of poverty in less developed countries which result in habitat transformations and losses of biological diversity .
	manualset3
155733	1	410367	13	NULL	NULL	0	NULL	human uterus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The human uterus undergoes profound physiological tissue remodelling during pregnancy .
	manualset3
155734	2	410367	13	NULL	NULL	NULL	NULL	physiological tissue remodelling	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The human uterus undergoes profound physiological tissue remodelling during pregnancy .
	manualset3
155735	3	410367	13	NULL	NULL	0	NULL	pregnancy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The human uterus undergoes profound physiological tissue remodelling during pregnancy .
	manualset3
155736	1	410368	13	NULL	NULL	0	NULL	telephone survey	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A telephone survey of primary care physicians in an area with a high incidence of STDs ( Washington , DC ) to ascertain the determinants and the extent of screening and counseling for STDs was completed in 1987 .
	manualset3
155737	2	410368	13	NULL	NULL	0	NULL	primary care physicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A telephone survey of primary care physicians in an area with a high incidence of STDs ( Washington , DC ) to ascertain the determinants and the extent of screening and counseling for STDs was completed in 1987 .
	manualset3
155738	3	410368	13	NULL	NULL	0	NULL	area 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A telephone survey of primary care physicians in an area with a high incidence of STDs ( Washington , DC ) to ascertain the determinants and the extent of screening and counseling for STDs was completed in 1987 .
	manualset3
155739	4	410368	13	NULL	NULL	0	NULL	incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A telephone survey of primary care physicians in an area with a high incidence of STDs ( Washington , DC ) to ascertain the determinants and the extent of screening and counseling for STDs was completed in 1987 .
	manualset3
155740	5	410368	13	NULL	NULL	0	NULL	STDs	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A telephone survey of primary care physicians in an area with a high incidence of STDs ( Washington , DC ) to ascertain the determinants and the extent of screening and counseling for STDs was completed in 1987 .
	manualset3
155741	6	410368	13	NULL	NULL	0	NULL	Washington , DC	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A telephone survey of primary care physicians in an area with a high incidence of STDs ( Washington , DC ) to ascertain the determinants and the extent of screening and counseling for STDs was completed in 1987 .
	manualset3
155742	7	410368	13	NULL	NULL	0	NULL	determinants 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A telephone survey of primary care physicians in an area with a high incidence of STDs ( Washington , DC ) to ascertain the determinants and the extent of screening and counseling for STDs was completed in 1987 .
	manualset3
155743	8	410368	13	NULL	NULL	0	NULL	extent	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A telephone survey of primary care physicians in an area with a high incidence of STDs ( Washington , DC ) to ascertain the determinants and the extent of screening and counseling for STDs was completed in 1987 .
	manualset3
155744	9	410368	13	NULL	NULL	0	NULL	screening 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A telephone survey of primary care physicians in an area with a high incidence of STDs ( Washington , DC ) to ascertain the determinants and the extent of screening and counseling for STDs was completed in 1987 .
	manualset3
155745	10	410368	13	NULL	NULL	0	NULL	counseling	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A telephone survey of primary care physicians in an area with a high incidence of STDs ( Washington , DC ) to ascertain the determinants and the extent of screening and counseling for STDs was completed in 1987 .
	manualset3
155746	11	410368	13	NULL	NULL	0	NULL	STDs	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A telephone survey of primary care physicians in an area with a high incidence of STDs ( Washington , DC ) to ascertain the determinants and the extent of screening and counseling for STDs was completed in 1987 .
	manualset3
155747	12	410368	13	NULL	NULL	0	NULL	1987	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	A telephone survey of primary care physicians in an area with a high incidence of STDs ( Washington , DC ) to ascertain the determinants and the extent of screening and counseling for STDs was completed in 1987 .
	manualset3
155748	1	410369	13	NULL	NULL	0	NULL	humoral study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The humoral study showed thrombocytosis , high levels of IL-1beta and IL-6 and of some coagulative/fibrinolytic and endothelial factors ( von Willebrand factor , plasmin-antiplasmine complexes , plasminogen activator ) .
	manualset3
155749	3	410369	13	NULL	NULL	NULL	NULL	levels	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The humoral study showed thrombocytosis , high levels of IL-1beta and IL-6 and of some coagulative/fibrinolytic and endothelial factors ( von Willebrand factor , plasmin-antiplasmine complexes , plasminogen activator ) .
	manualset3
155750	4	410369	13	NULL	NULL	NULL	NULL	IL-1beta	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The humoral study showed thrombocytosis , high levels of IL-1beta and IL-6 and of some coagulative/fibrinolytic and endothelial factors ( von Willebrand factor , plasmin-antiplasmine complexes , plasminogen activator ) .
	manualset3
155751	5	410369	13	NULL	NULL	NULL	NULL	IL-6	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The humoral study showed thrombocytosis , high levels of IL-1beta and IL-6 and of some coagulative/fibrinolytic and endothelial factors ( von Willebrand factor , plasmin-antiplasmine complexes , plasminogen activator ) .
	manualset3
155752	2	410369	13	NULL	NULL	NULL	NULL	 thrombocytosis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The humoral study showed thrombocytosis , high levels of IL-1beta and IL-6 and of some coagulative/fibrinolytic and endothelial factors ( von Willebrand factor , plasmin-antiplasmine complexes , plasminogen activator ) .
	manualset3
155753	6	410369	13	NULL	NULL	0	NULL	coagulative/fibrinolytic factors  	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The humoral study showed thrombocytosis , high levels of IL-1beta and IL-6 and of some coagulative/fibrinolytic and endothelial factors ( von Willebrand factor , plasmin-antiplasmine complexes , plasminogen activator ) .
	manualset3
155754	7	410369	13	NULL	NULL	0	NULL	endothelial factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The humoral study showed thrombocytosis , high levels of IL-1beta and IL-6 and of some coagulative/fibrinolytic and endothelial factors ( von Willebrand factor , plasmin-antiplasmine complexes , plasminogen activator ) .
	manualset3
155755	8	410369	13	NULL	NULL	0	NULL	Willebrand factor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The humoral study showed thrombocytosis , high levels of IL-1beta and IL-6 and of some coagulative/fibrinolytic and endothelial factors ( von Willebrand factor , plasmin-antiplasmine complexes , plasminogen activator ) .
	manualset3
155756	9	410369	13	NULL	NULL	0	NULL	plasmin-antiplasmine complexes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The humoral study showed thrombocytosis , high levels of IL-1beta and IL-6 and of some coagulative/fibrinolytic and endothelial factors ( von Willebrand factor , plasmin-antiplasmine complexes , plasminogen activator ) .
	manualset3
155757	10	410369	13	NULL	NULL	0	NULL	plasminogen activator	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The humoral study showed thrombocytosis , high levels of IL-1beta and IL-6 and of some coagulative/fibrinolytic and endothelial factors ( von Willebrand factor , plasmin-antiplasmine complexes , plasminogen activator ) .
	manualset3
155758	1	410370	13	NULL	NULL	0	NULL	hybrids	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The hybrids of the lymphocyte cell and mouse erythroleukemia cell ( MEL ) were achieved and the hybrids containing human chromosome 11 were selected with the monoclonal antibody 53/6 .
	manualset3
155759	2	410370	13	NULL	NULL	0	NULL	lymphocyte cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The hybrids of the lymphocyte cell and mouse erythroleukemia cell ( MEL ) were achieved and the hybrids containing human chromosome 11 were selected with the monoclonal antibody 53/6 .
	manualset3
155760	3	410370	13	NULL	NULL	0	NULL	mouse erythroleukemia cell ( MEL )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The hybrids of the lymphocyte cell and mouse erythroleukemia cell ( MEL ) were achieved and the hybrids containing human chromosome 11 were selected with the monoclonal antibody 53/6 .
	manualset3
155761	4	410370	13	NULL	NULL	0	NULL	hybrids	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The hybrids of the lymphocyte cell and mouse erythroleukemia cell ( MEL ) were achieved and the hybrids containing human chromosome 11 were selected with the monoclonal antibody 53/6 .
	manualset3
155762	5	410370	13	NULL	NULL	0	NULL	human chromosome 11 	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The hybrids of the lymphocyte cell and mouse erythroleukemia cell ( MEL ) were achieved and the hybrids containing human chromosome 11 were selected with the monoclonal antibody 53/6 .
	manualset3
155763	6	410370	13	NULL	NULL	0	NULL	monoclonal antibody 53/6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The hybrids of the lymphocyte cell and mouse erythroleukemia cell ( MEL ) were achieved and the hybrids containing human chromosome 11 were selected with the monoclonal antibody 53/6 .
	manualset3
155809	1	410371	13	NULL	NULL	0	NULL	hydrogels	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydrogels were formed by ionic association of the template molecule , GPS-Ba , to the polymer , prior to covalent crosslinking using epichlorohydrin ( EPI ) .
	manualset3
155810	2	410371	13	NULL	NULL	0	NULL	 ionic association	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydrogels were formed by ionic association of the template molecule , GPS-Ba , to the polymer , prior to covalent crosslinking using epichlorohydrin ( EPI ) .
	manualset3
155811	3	410371	13	NULL	NULL	0	NULL	template molecule	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydrogels were formed by ionic association of the template molecule , GPS-Ba , to the polymer , prior to covalent crosslinking using epichlorohydrin ( EPI ) .
	manualset3
155812	4	410371	13	NULL	NULL	0	NULL	 GPS-Ba	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydrogels were formed by ionic association of the template molecule , GPS-Ba , to the polymer , prior to covalent crosslinking using epichlorohydrin ( EPI ) .
	manualset3
155813	5	410371	13	NULL	NULL	0	NULL	polymer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydrogels were formed by ionic association of the template molecule , GPS-Ba , to the polymer , prior to covalent crosslinking using epichlorohydrin ( EPI ) .
	manualset3
155814	6	410371	13	NULL	NULL	0	NULL	 crosslinking	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydrogels were formed by ionic association of the template molecule , GPS-Ba , to the polymer , prior to covalent crosslinking using epichlorohydrin ( EPI ) .
	manualset3
155815	7	410371	13	NULL	NULL	0	NULL	epichlorohydrin ( EPI ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydrogels were formed by ionic association of the template molecule , GPS-Ba , to the polymer , prior to covalent crosslinking using epichlorohydrin ( EPI ) .
	manualset3
155816	1	410372	13	NULL	NULL	0	NULL	hydrogen-bond energies	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydrogen-bond and nonspecific interaction energies for 4-aminophthalimide ( 4-AP ) , often used as a probe , in the ground electronic and excited singlet states are determined using ab initio computational methods .
	manualset3
155817	2	410372	13	NULL	NULL	0	NULL	interaction energies	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydrogen-bond and nonspecific interaction energies for 4-aminophthalimide ( 4-AP ) , often used as a probe , in the ground electronic and excited singlet states are determined using ab initio computational methods .
	manualset3
155818	3	410372	13	NULL	NULL	0	NULL	 4-aminophthalimide ( 4-AP )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydrogen-bond and nonspecific interaction energies for 4-aminophthalimide ( 4-AP ) , often used as a probe , in the ground electronic and excited singlet states are determined using ab initio computational methods .
	manualset3
155819	4	410372	13	NULL	NULL	0	NULL	probe	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydrogen-bond and nonspecific interaction energies for 4-aminophthalimide ( 4-AP ) , often used as a probe , in the ground electronic and excited singlet states are determined using ab initio computational methods .
	manualset3
155820	5	410372	13	NULL	NULL	0	NULL	ground electronic states	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydrogen-bond and nonspecific interaction energies for 4-aminophthalimide ( 4-AP ) , often used as a probe , in the ground electronic and excited singlet states are determined using ab initio computational methods .
	manualset3
155821	6	410372	13	NULL	NULL	0	NULL	 excited singlet states	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydrogen-bond and nonspecific interaction energies for 4-aminophthalimide ( 4-AP ) , often used as a probe , in the ground electronic and excited singlet states are determined using ab initio computational methods .
	manualset3
155822	7	410372	13	NULL	NULL	0	NULL	ab initio computational methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydrogen-bond and nonspecific interaction energies for 4-aminophthalimide ( 4-AP ) , often used as a probe , in the ground electronic and excited singlet states are determined using ab initio computational methods .
	manualset3
155823	1	410373	13	NULL	NULL	0	NULL	hydrolysis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydrolysis of urea and the proficiency of urease .
	manualset3
155824	2	410373	13	NULL	NULL	0	NULL	urea	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydrolysis of urea and the proficiency of urease .
	manualset3
155825	3	410373	13	NULL	NULL	0	NULL	proficiency	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydrolysis of urea and the proficiency of urease .
	manualset3
155826	4	410373	13	NULL	NULL	0	NULL	urease	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydrolysis of urea and the proficiency of urease .
	manualset3
155827	1	410374	13	NULL	NULL	0	NULL	hydrophobicity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydrophobicity of the head groups of ADL6 , ADL8 and ADL10 is suitable as triggers of membrane fusion .
	manualset3
155828	2	410374	13	NULL	NULL	0	NULL	head groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydrophobicity of the head groups of ADL6 , ADL8 and ADL10 is suitable as triggers of membrane fusion .
	manualset3
155829	3	410374	13	NULL	NULL	0	NULL	ADL6	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydrophobicity of the head groups of ADL6 , ADL8 and ADL10 is suitable as triggers of membrane fusion .
	manualset3
155830	4	410374	13	NULL	NULL	0	NULL	ADL8	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydrophobicity of the head groups of ADL6 , ADL8 and ADL10 is suitable as triggers of membrane fusion .
	manualset3
155831	5	410374	13	NULL	NULL	0	NULL	ADL10	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydrophobicity of the head groups of ADL6 , ADL8 and ADL10 is suitable as triggers of membrane fusion .
	manualset3
155832	6	410374	13	NULL	NULL	0	NULL	triggers	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydrophobicity of the head groups of ADL6 , ADL8 and ADL10 is suitable as triggers of membrane fusion .
	manualset3
155833	7	410374	13	NULL	NULL	0	NULL	membrane fusion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydrophobicity of the head groups of ADL6 , ADL8 and ADL10 is suitable as triggers of membrane fusion .
	manualset3
155834	1	410375	13	NULL	NULL	0	NULL	hydroxylation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydroxylation of 7 alpha-hydroxycholesterol was similar in characteristics to cholesterol 7 alpha-hydroxylase activity in that it was dependent on NADPH , was inhibited by several known P450 inhibitors , and was affected by an inhibitory autobody elicited against rat hepatic NADPH : cytochrome P450 oxidoreductase .
	manualset3
155835	2	410375	13	NULL	NULL	0	NULL	7 alpha-hydroxycholesterol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydroxylation of 7 alpha-hydroxycholesterol was similar in characteristics to cholesterol 7 alpha-hydroxylase activity in that it was dependent on NADPH , was inhibited by several known P450 inhibitors , and was affected by an inhibitory autobody elicited against rat hepatic NADPH : cytochrome P450 oxidoreductase .
	manualset3
155836	3	410375	13	NULL	NULL	0	NULL	characteristics	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydroxylation of 7 alpha-hydroxycholesterol was similar in characteristics to cholesterol 7 alpha-hydroxylase activity in that it was dependent on NADPH , was inhibited by several known P450 inhibitors , and was affected by an inhibitory autobody elicited against rat hepatic NADPH : cytochrome P450 oxidoreductase .
	manualset3
155837	4	410375	13	NULL	NULL	0	NULL	cholesterol 7 alpha-hydroxylase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydroxylation of 7 alpha-hydroxycholesterol was similar in characteristics to cholesterol 7 alpha-hydroxylase activity in that it was dependent on NADPH , was inhibited by several known P450 inhibitors , and was affected by an inhibitory autobody elicited against rat hepatic NADPH : cytochrome P450 oxidoreductase .
	manualset3
155838	5	410375	13	NULL	NULL	0	NULL	NADPH 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydroxylation of 7 alpha-hydroxycholesterol was similar in characteristics to cholesterol 7 alpha-hydroxylase activity in that it was dependent on NADPH , was inhibited by several known P450 inhibitors , and was affected by an inhibitory autobody elicited against rat hepatic NADPH : cytochrome P450 oxidoreductase .
	manualset3
155839	6	410375	13	NULL	NULL	0	NULL	P450 inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydroxylation of 7 alpha-hydroxycholesterol was similar in characteristics to cholesterol 7 alpha-hydroxylase activity in that it was dependent on NADPH , was inhibited by several known P450 inhibitors , and was affected by an inhibitory autobody elicited against rat hepatic NADPH : cytochrome P450 oxidoreductase .
	manualset3
155840	7	410375	13	NULL	NULL	0	NULL	inhibitory autobody	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydroxylation of 7 alpha-hydroxycholesterol was similar in characteristics to cholesterol 7 alpha-hydroxylase activity in that it was dependent on NADPH , was inhibited by several known P450 inhibitors , and was affected by an inhibitory autobody elicited against rat hepatic NADPH : cytochrome P450 oxidoreductase .
	manualset3
155841	8	410375	13	NULL	NULL	0	NULL	rat hepatic NADPH : cytochrome P450 oxidoreductase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydroxylation of 7 alpha-hydroxycholesterol was similar in characteristics to cholesterol 7 alpha-hydroxylase activity in that it was dependent on NADPH , was inhibited by several known P450 inhibitors , and was affected by an inhibitory autobody elicited against rat hepatic NADPH : cytochrome P450 oxidoreductase .
	manualset3
155842	1	410376	13	NULL	NULL	0	NULL	hydroxyproline content	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydroxyproline content of regenerating tissue increased significantly 7 and 10 days after patching but was similar in the two groups ( 30.8 + / - 5.9 micrograms/mg tissue Day 10 vs 12.8 + / - 2.8 Day 1 ) .
	manualset3
155843	2	410376	13	NULL	NULL	0	NULL	 tissue 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydroxyproline content of regenerating tissue increased significantly 7 and 10 days after patching but was similar in the two groups ( 30.8 + / - 5.9 micrograms/mg tissue Day 10 vs 12.8 + / - 2.8 Day 1 ) .
	manualset3
155844	3	410376	13	NULL	NULL	0	NULL	7 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydroxyproline content of regenerating tissue increased significantly 7 and 10 days after patching but was similar in the two groups ( 30.8 + / - 5.9 micrograms/mg tissue Day 10 vs 12.8 + / - 2.8 Day 1 ) .
	manualset3
155845	4	410376	13	NULL	NULL	0	NULL	10 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydroxyproline content of regenerating tissue increased significantly 7 and 10 days after patching but was similar in the two groups ( 30.8 + / - 5.9 micrograms/mg tissue Day 10 vs 12.8 + / - 2.8 Day 1 ) .
	manualset3
155846	5	410376	13	NULL	NULL	0	NULL	two groups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydroxyproline content of regenerating tissue increased significantly 7 and 10 days after patching but was similar in the two groups ( 30.8 + / - 5.9 micrograms/mg tissue Day 10 vs 12.8 + / - 2.8 Day 1 ) .
	manualset3
155847	6	410376	13	NULL	NULL	0	NULL	30.8 + / - 5.9 micrograms/mg tissue Day 10 vs 12.8 + / - 2.8 Day 1 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydroxyproline content of regenerating tissue increased significantly 7 and 10 days after patching but was similar in the two groups ( 30.8 + / - 5.9 micrograms/mg tissue Day 10 vs 12.8 + / - 2.8 Day 1 ) .
	manualset3
155848	1	410377	13	NULL	NULL	0	NULL	hypercoagulable state	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypercoagulable state refers to those factors , both acquired and congenital , that predispose an individual to thromboembolic events .
	manualset3
155849	2	410377	13	NULL	NULL	0	NULL	factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypercoagulable state refers to those factors , both acquired and congenital , that predispose an individual to thromboembolic events .
	manualset3
155850	3	410377	13	NULL	NULL	0	NULL	thromboembolic events	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypercoagulable state refers to those factors , both acquired and congenital , that predispose an individual to thromboembolic events .
	manualset3
155851	1	410378	13	NULL	NULL	0	NULL	temperature	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A temperature reduction of 6 degrees C had no impact on the removal of free estrogens , but removal of the conjugated estrone-3-sulfate was reduced by 20 % .
	manualset3
155852	2	410378	13	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A temperature reduction of 6 degrees C had no impact on the removal of free estrogens , but removal of the conjugated estrone-3-sulfate was reduced by 20 % .
	manualset3
155853	3	410378	13	NULL	NULL	0	NULL	6 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A temperature reduction of 6 degrees C had no impact on the removal of free estrogens , but removal of the conjugated estrone-3-sulfate was reduced by 20 % .
	manualset3
155854	4	410378	13	NULL	NULL	0	NULL	impact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A temperature reduction of 6 degrees C had no impact on the removal of free estrogens , but removal of the conjugated estrone-3-sulfate was reduced by 20 % .
	manualset3
155855	5	410378	13	NULL	NULL	0	NULL	removal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A temperature reduction of 6 degrees C had no impact on the removal of free estrogens , but removal of the conjugated estrone-3-sulfate was reduced by 20 % .
	manualset3
155856	6	410378	13	NULL	NULL	0	NULL	free estrogens 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A temperature reduction of 6 degrees C had no impact on the removal of free estrogens , but removal of the conjugated estrone-3-sulfate was reduced by 20 % .
	manualset3
155857	7	410378	13	NULL	NULL	0	NULL	removal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A temperature reduction of 6 degrees C had no impact on the removal of free estrogens , but removal of the conjugated estrone-3-sulfate was reduced by 20 % .
	manualset3
155858	8	410378	13	NULL	NULL	0	NULL	 estrone-3-sulfate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A temperature reduction of 6 degrees C had no impact on the removal of free estrogens , but removal of the conjugated estrone-3-sulfate was reduced by 20 % .
	manualset3
155859	9	410378	13	NULL	NULL	0	NULL	20 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A temperature reduction of 6 degrees C had no impact on the removal of free estrogens , but removal of the conjugated estrone-3-sulfate was reduced by 20 % .
	manualset3
155860	1	410379	13	NULL	NULL	0	NULL	hyperdynamic circulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The hyperdynamic circulation may be necessary to meet increased tissue delivery requirements for O2 and amino acids .
	manualset3
155861	2	410379	13	NULL	NULL	0	NULL	tissue 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The hyperdynamic circulation may be necessary to meet increased tissue delivery requirements for O2 and amino acids .
	manualset3
155862	3	410379	13	NULL	NULL	0	NULL	delivery requirements	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The hyperdynamic circulation may be necessary to meet increased tissue delivery requirements for O2 and amino acids .
	manualset3
155863	4	410379	13	NULL	NULL	0	NULL	O2 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The hyperdynamic circulation may be necessary to meet increased tissue delivery requirements for O2 and amino acids .
	manualset3
155864	5	410379	13	NULL	NULL	0	NULL	amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The hyperdynamic circulation may be necessary to meet increased tissue delivery requirements for O2 and amino acids .
	manualset3
155865	1	410380	13	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The hyperpolarizing effect of noradrenaline ( 30 microM ) was potentiated in the presence of ( - ) - tramadol ( 100 microM ) , but not in the presence of ( + ) - O-desmethyltramadol ( 10 microM ) .
	manualset3
155866	2	410380	13	NULL	NULL	NULL	NULL	noradrenaline	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The hyperpolarizing effect of noradrenaline ( 30 microM ) was potentiated in the presence of ( - ) - tramadol ( 100 microM ) , but not in the presence of ( + ) - O-desmethyltramadol ( 10 microM ) .
	manualset3
155867	3	410380	13	NULL	NULL	0	NULL	30 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The hyperpolarizing effect of noradrenaline ( 30 microM ) was potentiated in the presence of ( - ) - tramadol ( 100 microM ) , but not in the presence of ( + ) - O-desmethyltramadol ( 10 microM ) .
	manualset3
155868	4	410380	13	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The hyperpolarizing effect of noradrenaline ( 30 microM ) was potentiated in the presence of ( - ) - tramadol ( 100 microM ) , but not in the presence of ( + ) - O-desmethyltramadol ( 10 microM ) .
	manualset3
155869	5	410380	13	NULL	NULL	0	NULL	 tramadol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The hyperpolarizing effect of noradrenaline ( 30 microM ) was potentiated in the presence of ( - ) - tramadol ( 100 microM ) , but not in the presence of ( + ) - O-desmethyltramadol ( 10 microM ) .
	manualset3
155870	6	410380	13	NULL	NULL	0	NULL	100 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The hyperpolarizing effect of noradrenaline ( 30 microM ) was potentiated in the presence of ( - ) - tramadol ( 100 microM ) , but not in the presence of ( + ) - O-desmethyltramadol ( 10 microM ) .
	manualset3
155871	7	410380	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The hyperpolarizing effect of noradrenaline ( 30 microM ) was potentiated in the presence of ( - ) - tramadol ( 100 microM ) , but not in the presence of ( + ) - O-desmethyltramadol ( 10 microM ) .
	manualset3
155872	8	410380	13	NULL	NULL	0	NULL	O-desmethyltramadol 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The hyperpolarizing effect of noradrenaline ( 30 microM ) was potentiated in the presence of ( - ) - tramadol ( 100 microM ) , but not in the presence of ( + ) - O-desmethyltramadol ( 10 microM ) .
	manualset3
155873	9	410380	13	NULL	NULL	0	NULL	 10 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The hyperpolarizing effect of noradrenaline ( 30 microM ) was potentiated in the presence of ( - ) - tramadol ( 100 microM ) , but not in the presence of ( + ) - O-desmethyltramadol ( 10 microM ) .
	manualset3
155874	1	410381	13	NULL	NULL	0	NULL	T residue 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The hyperreactive T residue in the six sites detected as well as the one in Fragment 67 and three in the 5 S rDNA positioning sequence were contained within a TA step .
	manualset3
155875	2	410381	13	NULL	NULL	0	NULL	six sites	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The hyperreactive T residue in the six sites detected as well as the one in Fragment 67 and three in the 5 S rDNA positioning sequence were contained within a TA step .
	manualset3
155876	3	410381	13	NULL	NULL	0	NULL	Fragment 67	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The hyperreactive T residue in the six sites detected as well as the one in Fragment 67 and three in the 5 S rDNA positioning sequence were contained within a TA step .
	manualset3
155877	4	410381	13	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The hyperreactive T residue in the six sites detected as well as the one in Fragment 67 and three in the 5 S rDNA positioning sequence were contained within a TA step .
	manualset3
155878	5	410381	13	NULL	NULL	0	NULL	5 S rDNA positioning sequence 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The hyperreactive T residue in the six sites detected as well as the one in Fragment 67 and three in the 5 S rDNA positioning sequence were contained within a TA step .
	manualset3
155879	6	410381	13	NULL	NULL	0	NULL	TA step 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The hyperreactive T residue in the six sites detected as well as the one in Fragment 67 and three in the 5 S rDNA positioning sequence were contained within a TA step .
	manualset3
155880	1	410382	13	NULL	NULL	0	NULL	hypoglycemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypoglycemia elicited a significant rise in serum PG I on both days .
	manualset3
155881	2	410382	13	NULL	NULL	NULL	NULL	rise 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The hypoglycemia elicited a significant rise in serum PG I on both days .
	manualset3
155882	3	410382	13	NULL	NULL	0	NULL	serum PG I	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypoglycemia elicited a significant rise in serum PG I on both days .
	manualset3
155883	4	410382	13	NULL	NULL	0	NULL	both days	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypoglycemia elicited a significant rise in serum PG I on both days .
	manualset3
155884	1	410383	13	NULL	NULL	0	NULL	 hypotheses	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypotheses were tested by coupling calcium kinetics with XB cycling .
	manualset3
155885	2	410383	13	NULL	NULL	0	NULL	calcium kinetics	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypotheses were tested by coupling calcium kinetics with XB cycling .
	manualset3
155886	3	410383	13	NULL	NULL	0	NULL	XB cycling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypotheses were tested by coupling calcium kinetics with XB cycling .
	manualset3
155887	1	410384	13	NULL	NULL	0	NULL	 hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis in this study was that slow psychomotor reaction time is related to low-back pain .
	manualset3
155888	2	410384	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis in this study was that slow psychomotor reaction time is related to low-back pain .
	manualset3
155889	3	410384	13	NULL	NULL	0	NULL	psychomotor reaction time	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis in this study was that slow psychomotor reaction time is related to low-back pain .
	manualset3
155890	4	410384	13	NULL	NULL	0	NULL	low-back pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis in this study was that slow psychomotor reaction time is related to low-back pain .
	manualset3
155891	1	410385	13	NULL	NULL	0	NULL	hypothesis 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis is that if clinicians indeed interpret the SpHb values as macro hemoglobin values then there is an unreported discrepancy between SpHb to macro hemoglobin concentrations during blood loss due to the increasing effect of microcirculatory hemoglobin measurement on the mixed parameter , SpHb .
	manualset3
155892	2	410385	13	NULL	NULL	0	NULL	clinicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis is that if clinicians indeed interpret the SpHb values as macro hemoglobin values then there is an unreported discrepancy between SpHb to macro hemoglobin concentrations during blood loss due to the increasing effect of microcirculatory hemoglobin measurement on the mixed parameter , SpHb .
	manualset3
155893	3	410385	13	NULL	NULL	0	NULL	SpHb values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis is that if clinicians indeed interpret the SpHb values as macro hemoglobin values then there is an unreported discrepancy between SpHb to macro hemoglobin concentrations during blood loss due to the increasing effect of microcirculatory hemoglobin measurement on the mixed parameter , SpHb .
	manualset3
155894	4	410385	13	NULL	NULL	0	NULL	macro hemoglobin values 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis is that if clinicians indeed interpret the SpHb values as macro hemoglobin values then there is an unreported discrepancy between SpHb to macro hemoglobin concentrations during blood loss due to the increasing effect of microcirculatory hemoglobin measurement on the mixed parameter , SpHb .
	manualset3
155895	5	410385	13	NULL	NULL	0	NULL	discrepancy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis is that if clinicians indeed interpret the SpHb values as macro hemoglobin values then there is an unreported discrepancy between SpHb to macro hemoglobin concentrations during blood loss due to the increasing effect of microcirculatory hemoglobin measurement on the mixed parameter , SpHb .
	manualset3
155896	6	410385	13	NULL	NULL	0	NULL	SpHb concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis is that if clinicians indeed interpret the SpHb values as macro hemoglobin values then there is an unreported discrepancy between SpHb to macro hemoglobin concentrations during blood loss due to the increasing effect of microcirculatory hemoglobin measurement on the mixed parameter , SpHb .
	manualset3
155897	7	410385	13	NULL	NULL	0	NULL	macro hemoglobin concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis is that if clinicians indeed interpret the SpHb values as macro hemoglobin values then there is an unreported discrepancy between SpHb to macro hemoglobin concentrations during blood loss due to the increasing effect of microcirculatory hemoglobin measurement on the mixed parameter , SpHb .
	manualset3
155898	8	410385	13	NULL	NULL	0	NULL	blood loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis is that if clinicians indeed interpret the SpHb values as macro hemoglobin values then there is an unreported discrepancy between SpHb to macro hemoglobin concentrations during blood loss due to the increasing effect of microcirculatory hemoglobin measurement on the mixed parameter , SpHb .
	manualset3
155899	9	410385	13	NULL	NULL	0	NULL	effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis is that if clinicians indeed interpret the SpHb values as macro hemoglobin values then there is an unreported discrepancy between SpHb to macro hemoglobin concentrations during blood loss due to the increasing effect of microcirculatory hemoglobin measurement on the mixed parameter , SpHb .
	manualset3
155900	10	410385	13	NULL	NULL	0	NULL	microcirculatory hemoglobin measurement	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis is that if clinicians indeed interpret the SpHb values as macro hemoglobin values then there is an unreported discrepancy between SpHb to macro hemoglobin concentrations during blood loss due to the increasing effect of microcirculatory hemoglobin measurement on the mixed parameter , SpHb .
	manualset3
155901	11	410385	13	NULL	NULL	0	NULL	parameter	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis is that if clinicians indeed interpret the SpHb values as macro hemoglobin values then there is an unreported discrepancy between SpHb to macro hemoglobin concentrations during blood loss due to the increasing effect of microcirculatory hemoglobin measurement on the mixed parameter , SpHb .
	manualset3
155902	12	410385	13	NULL	NULL	0	NULL	SpHb	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis is that if clinicians indeed interpret the SpHb values as macro hemoglobin values then there is an unreported discrepancy between SpHb to macro hemoglobin concentrations during blood loss due to the increasing effect of microcirculatory hemoglobin measurement on the mixed parameter , SpHb .
	manualset3
155903	1	410386	13	NULL	NULL	0	NULL	hypothesis 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis of the current investigation was that CO2-exposure with subsequent CO2 removal would be beneficial during short-term chinook salmon milt storage .
	manualset3
155904	2	410386	13	NULL	NULL	0	NULL	investigation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis of the current investigation was that CO2-exposure with subsequent CO2 removal would be beneficial during short-term chinook salmon milt storage .
	manualset3
155905	3	410386	13	NULL	NULL	0	NULL	CO2-exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis of the current investigation was that CO2-exposure with subsequent CO2 removal would be beneficial during short-term chinook salmon milt storage .
	manualset3
155906	4	410386	13	NULL	NULL	0	NULL	CO2 removal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis of the current investigation was that CO2-exposure with subsequent CO2 removal would be beneficial during short-term chinook salmon milt storage .
	manualset3
155907	5	410386	13	NULL	NULL	0	NULL	chinook salmon	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis of the current investigation was that CO2-exposure with subsequent CO2 removal would be beneficial during short-term chinook salmon milt storage .
	manualset3
155908	6	410386	13	NULL	NULL	0	NULL	milt	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis of the current investigation was that CO2-exposure with subsequent CO2 removal would be beneficial during short-term chinook salmon milt storage .
	manualset3
155909	7	410386	13	NULL	NULL	0	NULL	storage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis of the current investigation was that CO2-exposure with subsequent CO2 removal would be beneficial during short-term chinook salmon milt storage .
	manualset3
155910	1	410387	13	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis that catheter-related sepsis ( CRS ) may be preceded by contamination of the catheter hub was tested in neonates with central venous catheters .
	manualset3
155911	2	410387	13	NULL	NULL	0	NULL	 catheter-related sepsis ( CRS ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis that catheter-related sepsis ( CRS ) may be preceded by contamination of the catheter hub was tested in neonates with central venous catheters .
	manualset3
155912	3	410387	13	NULL	NULL	0	NULL	contamination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis that catheter-related sepsis ( CRS ) may be preceded by contamination of the catheter hub was tested in neonates with central venous catheters .
	manualset3
155913	4	410387	13	NULL	NULL	0	NULL	catheter hub	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis that catheter-related sepsis ( CRS ) may be preceded by contamination of the catheter hub was tested in neonates with central venous catheters .
	manualset3
155914	5	410387	13	NULL	NULL	0	NULL	neonates	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis that catheter-related sepsis ( CRS ) may be preceded by contamination of the catheter hub was tested in neonates with central venous catheters .
	manualset3
155915	6	410387	13	NULL	NULL	0	NULL	 central venous catheters	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis that catheter-related sepsis ( CRS ) may be preceded by contamination of the catheter hub was tested in neonates with central venous catheters .
	manualset3
155916	1	410388	13	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis that the relaxant action of many drugs on vascular and other smooth muscle is mediated by increases in intracellular cGMP , the `` cGMP hypothesis , '' is gaining wide acceptance .
	manualset3
155917	2	410388	13	NULL	NULL	0	NULL	relaxant action	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis that the relaxant action of many drugs on vascular and other smooth muscle is mediated by increases in intracellular cGMP , the `` cGMP hypothesis , '' is gaining wide acceptance .
	manualset3
155918	3	410388	13	NULL	NULL	0	NULL	drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis that the relaxant action of many drugs on vascular and other smooth muscle is mediated by increases in intracellular cGMP , the `` cGMP hypothesis , '' is gaining wide acceptance .
	manualset3
155919	4	410388	13	NULL	NULL	0	NULL	vascular muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis that the relaxant action of many drugs on vascular and other smooth muscle is mediated by increases in intracellular cGMP , the `` cGMP hypothesis , '' is gaining wide acceptance .
	manualset3
155920	5	410388	13	NULL	NULL	0	NULL	smooth muscle 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis that the relaxant action of many drugs on vascular and other smooth muscle is mediated by increases in intracellular cGMP , the `` cGMP hypothesis , '' is gaining wide acceptance .
	manualset3
155921	6	410388	13	NULL	NULL	0	NULL	increases	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis that the relaxant action of many drugs on vascular and other smooth muscle is mediated by increases in intracellular cGMP , the `` cGMP hypothesis , '' is gaining wide acceptance .
	manualset3
155922	7	410388	13	NULL	NULL	0	NULL	 intracellular cGMP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis that the relaxant action of many drugs on vascular and other smooth muscle is mediated by increases in intracellular cGMP , the `` cGMP hypothesis , '' is gaining wide acceptance .
	manualset3
155923	8	410388	13	NULL	NULL	0	NULL	cGMP hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis that the relaxant action of many drugs on vascular and other smooth muscle is mediated by increases in intracellular cGMP , the `` cGMP hypothesis , '' is gaining wide acceptance .
	manualset3
155924	9	410388	13	NULL	NULL	0	NULL	acceptance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis that the relaxant action of many drugs on vascular and other smooth muscle is mediated by increases in intracellular cGMP , the `` cGMP hypothesis , '' is gaining wide acceptance .
	manualset3
155925	1	410389	13	NULL	NULL	0	NULL	Clinical notes 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical and therapeutic notes on 90 cases of influenza hospitalized in the Ospedale Maggiore of Cremona ( isolation ward : from October 1 to November 8 , 1957 ) ) .
	manualset3
155926	2	410389	13	NULL	NULL	0	NULL	therapeutic notes	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical and therapeutic notes on 90 cases of influenza hospitalized in the Ospedale Maggiore of Cremona ( isolation ward : from October 1 to November 8 , 1957 ) ) .
	manualset3
155927	3	410389	13	NULL	NULL	0	NULL	90 cases	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical and therapeutic notes on 90 cases of influenza hospitalized in the Ospedale Maggiore of Cremona ( isolation ward : from October 1 to November 8 , 1957 ) ) .
	manualset3
155928	4	410389	13	NULL	NULL	0	NULL	influenza	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical and therapeutic notes on 90 cases of influenza hospitalized in the Ospedale Maggiore of Cremona ( isolation ward : from October 1 to November 8 , 1957 ) ) .
	manualset3
155929	5	410389	13	NULL	NULL	0	NULL	Ospedale Maggiore	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical and therapeutic notes on 90 cases of influenza hospitalized in the Ospedale Maggiore of Cremona ( isolation ward : from October 1 to November 8 , 1957 ) ) .
	manualset3
155930	6	410389	13	NULL	NULL	0	NULL	Cremona	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical and therapeutic notes on 90 cases of influenza hospitalized in the Ospedale Maggiore of Cremona ( isolation ward : from October 1 to November 8 , 1957 ) ) .
	manualset3
155931	7	410389	13	NULL	NULL	0	NULL	isolation ward 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical and therapeutic notes on 90 cases of influenza hospitalized in the Ospedale Maggiore of Cremona ( isolation ward : from October 1 to November 8 , 1957 ) ) .
	manualset3
155932	8	410389	13	NULL	NULL	0	NULL	October 1 to November 8 , 1957 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical and therapeutic notes on 90 cases of influenza hospitalized in the Ospedale Maggiore of Cremona ( isolation ward : from October 1 to November 8 , 1957 ) ) .
	manualset3
155933	1	410390	13	NULL	NULL	0	NULL	temporal relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A temporal relation between the appearance of the discharge and vaginal exposure to topical spermicidal agents was determined .
	manualset3
155934	2	410390	13	NULL	NULL	0	NULL	appearance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A temporal relation between the appearance of the discharge and vaginal exposure to topical spermicidal agents was determined .
	manualset3
155935	3	410390	13	NULL	NULL	0	NULL	discharge 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A temporal relation between the appearance of the discharge and vaginal exposure to topical spermicidal agents was determined .
	manualset3
155936	4	410390	13	NULL	NULL	0	NULL	vaginal exposure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A temporal relation between the appearance of the discharge and vaginal exposure to topical spermicidal agents was determined .
	manualset3
155937	5	410390	13	NULL	NULL	0	NULL	topical spermicidal agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A temporal relation between the appearance of the discharge and vaginal exposure to topical spermicidal agents was determined .
	manualset3
155938	1	410391	13	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis was that the vastus lateralis ( VL ) and vastus medialis ( VM ) have significant off-axis moment arms compared to the central quadriceps components .
	manualset3
155939	2	410391	13	NULL	NULL	0	NULL	vastus lateralis ( VL )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis was that the vastus lateralis ( VL ) and vastus medialis ( VM ) have significant off-axis moment arms compared to the central quadriceps components .
	manualset3
155940	3	410391	13	NULL	NULL	0	NULL	vastus medialis ( VM ) 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis was that the vastus lateralis ( VL ) and vastus medialis ( VM ) have significant off-axis moment arms compared to the central quadriceps components .
	manualset3
155941	4	410391	13	NULL	NULL	0	NULL	off-axis moment arms	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis was that the vastus lateralis ( VL ) and vastus medialis ( VM ) have significant off-axis moment arms compared to the central quadriceps components .
	manualset3
155942	5	410391	13	NULL	NULL	0	NULL	central quadriceps components 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis was that the vastus lateralis ( VL ) and vastus medialis ( VM ) have significant off-axis moment arms compared to the central quadriceps components .
	manualset3
155943	1	410392	13	NULL	NULL	0	NULL	administration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The i.p. administration of rMuIFN-gamma to C57BL/6 mice at the time of TPA treatment , at doses that were co-promoting in SENCAR mice , did not increase papilloma multiplicities .
	manualset3
155944	2	410392	13	NULL	NULL	0	NULL	rMuIFN-gamma	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The i.p. administration of rMuIFN-gamma to C57BL/6 mice at the time of TPA treatment , at doses that were co-promoting in SENCAR mice , did not increase papilloma multiplicities .
	manualset3
155945	3	410392	13	NULL	NULL	0	NULL	C57BL/6 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The i.p. administration of rMuIFN-gamma to C57BL/6 mice at the time of TPA treatment , at doses that were co-promoting in SENCAR mice , did not increase papilloma multiplicities .
	manualset3
155946	4	410392	13	NULL	NULL	0	NULL	 time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The i.p. administration of rMuIFN-gamma to C57BL/6 mice at the time of TPA treatment , at doses that were co-promoting in SENCAR mice , did not increase papilloma multiplicities .
	manualset3
155947	5	410392	13	NULL	NULL	0	NULL	TPA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The i.p. administration of rMuIFN-gamma to C57BL/6 mice at the time of TPA treatment , at doses that were co-promoting in SENCAR mice , did not increase papilloma multiplicities .
	manualset3
155948	6	410392	13	NULL	NULL	0	NULL	treatment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The i.p. administration of rMuIFN-gamma to C57BL/6 mice at the time of TPA treatment , at doses that were co-promoting in SENCAR mice , did not increase papilloma multiplicities .
	manualset3
155949	7	410392	13	NULL	NULL	0	NULL	doses	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The i.p. administration of rMuIFN-gamma to C57BL/6 mice at the time of TPA treatment , at doses that were co-promoting in SENCAR mice , did not increase papilloma multiplicities .
	manualset3
155950	8	410392	13	NULL	NULL	0	NULL	SENCAR mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The i.p. administration of rMuIFN-gamma to C57BL/6 mice at the time of TPA treatment , at doses that were co-promoting in SENCAR mice , did not increase papilloma multiplicities .
	manualset3
155951	9	410392	13	NULL	NULL	0	NULL	papilloma multiplicities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The i.p. administration of rMuIFN-gamma to C57BL/6 mice at the time of TPA treatment , at doses that were co-promoting in SENCAR mice , did not increase papilloma multiplicities .
	manualset3
155952	1	410393	13	NULL	NULL	0	NULL	ideal position	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The ideal position was defined as that in which the carina was located at the same level with the middle 5 mm between the proximal margin of the endobronchial balloon and the circumferential black mark .
	manualset3
155953	2	410393	13	NULL	NULL	0	NULL	carina	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The ideal position was defined as that in which the carina was located at the same level with the middle 5 mm between the proximal margin of the endobronchial balloon and the circumferential black mark .
	manualset3
155954	3	410393	13	NULL	NULL	0	NULL	level	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ideal position was defined as that in which the carina was located at the same level with the middle 5 mm between the proximal margin of the endobronchial balloon and the circumferential black mark .
	manualset3
155955	4	410393	13	NULL	NULL	0	NULL	 5 mm 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ideal position was defined as that in which the carina was located at the same level with the middle 5 mm between the proximal margin of the endobronchial balloon and the circumferential black mark .
	manualset3
155956	5	410393	13	NULL	NULL	0	NULL	proximal margin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The ideal position was defined as that in which the carina was located at the same level with the middle 5 mm between the proximal margin of the endobronchial balloon and the circumferential black mark .
	manualset3
155957	6	410393	13	NULL	NULL	0	NULL	endobronchial balloon	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The ideal position was defined as that in which the carina was located at the same level with the middle 5 mm between the proximal margin of the endobronchial balloon and the circumferential black mark .
	manualset3
155958	7	410393	13	NULL	NULL	0	NULL	circumferential black mark 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The ideal position was defined as that in which the carina was located at the same level with the middle 5 mm between the proximal margin of the endobronchial balloon and the circumferential black mark .
	manualset3
155959	1	410394	13	NULL	NULL	0	NULL	identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification and molecular cloning of a target antigen , a glutathione S-transferase ( GST ) , has made it possible to demonstrate its vaccine potential in several animal species ( rodents , cattle , primates ) and to establish consistently the capacity of vaccination to reduce female worm fecundity and egg viability through the production of neutralizing antibodies ( IgA and IgG ) .
	manualset3
155960	2	410394	13	NULL	NULL	0	NULL	molecular cloning	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification and molecular cloning of a target antigen , a glutathione S-transferase ( GST ) , has made it possible to demonstrate its vaccine potential in several animal species ( rodents , cattle , primates ) and to establish consistently the capacity of vaccination to reduce female worm fecundity and egg viability through the production of neutralizing antibodies ( IgA and IgG ) .
	manualset3
155961	3	410394	13	NULL	NULL	0	NULL	target antigen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification and molecular cloning of a target antigen , a glutathione S-transferase ( GST ) , has made it possible to demonstrate its vaccine potential in several animal species ( rodents , cattle , primates ) and to establish consistently the capacity of vaccination to reduce female worm fecundity and egg viability through the production of neutralizing antibodies ( IgA and IgG ) .
	manualset3
155962	4	410394	13	NULL	NULL	0	NULL	glutathione S-transferase ( GST )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification and molecular cloning of a target antigen , a glutathione S-transferase ( GST ) , has made it possible to demonstrate its vaccine potential in several animal species ( rodents , cattle , primates ) and to establish consistently the capacity of vaccination to reduce female worm fecundity and egg viability through the production of neutralizing antibodies ( IgA and IgG ) .
	manualset3
155963	5	410394	13	NULL	NULL	0	NULL	vaccine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification and molecular cloning of a target antigen , a glutathione S-transferase ( GST ) , has made it possible to demonstrate its vaccine potential in several animal species ( rodents , cattle , primates ) and to establish consistently the capacity of vaccination to reduce female worm fecundity and egg viability through the production of neutralizing antibodies ( IgA and IgG ) .
	manualset3
155964	6	410394	13	NULL	NULL	0	NULL	several animal species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification and molecular cloning of a target antigen , a glutathione S-transferase ( GST ) , has made it possible to demonstrate its vaccine potential in several animal species ( rodents , cattle , primates ) and to establish consistently the capacity of vaccination to reduce female worm fecundity and egg viability through the production of neutralizing antibodies ( IgA and IgG ) .
	manualset3
155965	7	410394	13	NULL	NULL	0	NULL	rodents	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification and molecular cloning of a target antigen , a glutathione S-transferase ( GST ) , has made it possible to demonstrate its vaccine potential in several animal species ( rodents , cattle , primates ) and to establish consistently the capacity of vaccination to reduce female worm fecundity and egg viability through the production of neutralizing antibodies ( IgA and IgG ) .
	manualset3
155966	8	410394	13	NULL	NULL	0	NULL	cattle	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification and molecular cloning of a target antigen , a glutathione S-transferase ( GST ) , has made it possible to demonstrate its vaccine potential in several animal species ( rodents , cattle , primates ) and to establish consistently the capacity of vaccination to reduce female worm fecundity and egg viability through the production of neutralizing antibodies ( IgA and IgG ) .
	manualset3
155967	9	410394	13	NULL	NULL	0	NULL	primates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification and molecular cloning of a target antigen , a glutathione S-transferase ( GST ) , has made it possible to demonstrate its vaccine potential in several animal species ( rodents , cattle , primates ) and to establish consistently the capacity of vaccination to reduce female worm fecundity and egg viability through the production of neutralizing antibodies ( IgA and IgG ) .
	manualset3
155968	10	410394	13	NULL	NULL	0	NULL	capacity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification and molecular cloning of a target antigen , a glutathione S-transferase ( GST ) , has made it possible to demonstrate its vaccine potential in several animal species ( rodents , cattle , primates ) and to establish consistently the capacity of vaccination to reduce female worm fecundity and egg viability through the production of neutralizing antibodies ( IgA and IgG ) .
	manualset3
155969	11	410394	13	NULL	NULL	0	NULL	vaccination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification and molecular cloning of a target antigen , a glutathione S-transferase ( GST ) , has made it possible to demonstrate its vaccine potential in several animal species ( rodents , cattle , primates ) and to establish consistently the capacity of vaccination to reduce female worm fecundity and egg viability through the production of neutralizing antibodies ( IgA and IgG ) .
	manualset3
155970	12	410394	13	NULL	NULL	0	NULL	female worm fecundity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification and molecular cloning of a target antigen , a glutathione S-transferase ( GST ) , has made it possible to demonstrate its vaccine potential in several animal species ( rodents , cattle , primates ) and to establish consistently the capacity of vaccination to reduce female worm fecundity and egg viability through the production of neutralizing antibodies ( IgA and IgG ) .
	manualset3
155971	13	410394	13	NULL	NULL	0	NULL	egg viability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification and molecular cloning of a target antigen , a glutathione S-transferase ( GST ) , has made it possible to demonstrate its vaccine potential in several animal species ( rodents , cattle , primates ) and to establish consistently the capacity of vaccination to reduce female worm fecundity and egg viability through the production of neutralizing antibodies ( IgA and IgG ) .
	manualset3
155972	14	410394	13	NULL	NULL	0	NULL	production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification and molecular cloning of a target antigen , a glutathione S-transferase ( GST ) , has made it possible to demonstrate its vaccine potential in several animal species ( rodents , cattle , primates ) and to establish consistently the capacity of vaccination to reduce female worm fecundity and egg viability through the production of neutralizing antibodies ( IgA and IgG ) .
	manualset3
155973	15	410394	13	NULL	NULL	0	NULL	neutralizing antibodies 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification and molecular cloning of a target antigen , a glutathione S-transferase ( GST ) , has made it possible to demonstrate its vaccine potential in several animal species ( rodents , cattle , primates ) and to establish consistently the capacity of vaccination to reduce female worm fecundity and egg viability through the production of neutralizing antibodies ( IgA and IgG ) .
	manualset3
155974	16	410394	13	NULL	NULL	0	NULL	IgA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification and molecular cloning of a target antigen , a glutathione S-transferase ( GST ) , has made it possible to demonstrate its vaccine potential in several animal species ( rodents , cattle , primates ) and to establish consistently the capacity of vaccination to reduce female worm fecundity and egg viability through the production of neutralizing antibodies ( IgA and IgG ) .
	manualset3
155975	17	410394	13	NULL	NULL	0	NULL	IgG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification and molecular cloning of a target antigen , a glutathione S-transferase ( GST ) , has made it possible to demonstrate its vaccine potential in several animal species ( rodents , cattle , primates ) and to establish consistently the capacity of vaccination to reduce female worm fecundity and egg viability through the production of neutralizing antibodies ( IgA and IgG ) .
	manualset3
155976	1	410395	13	NULL	NULL	0	NULL	identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of a common mutation , delta F508 , in the CFTR gene allowed , for the first time , the detection of cystic fibrosis ( CF ) carriers in the general population .
	manualset3
155977	2	410395	13	NULL	NULL	0	NULL	mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of a common mutation , delta F508 , in the CFTR gene allowed , for the first time , the detection of cystic fibrosis ( CF ) carriers in the general population .
	manualset3
155978	3	410395	13	NULL	NULL	0	NULL	delta F508	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of a common mutation , delta F508 , in the CFTR gene allowed , for the first time , the detection of cystic fibrosis ( CF ) carriers in the general population .
	manualset3
155979	4	410395	13	NULL	NULL	0	NULL	CFTR gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of a common mutation , delta F508 , in the CFTR gene allowed , for the first time , the detection of cystic fibrosis ( CF ) carriers in the general population .
	manualset3
155980	5	410395	13	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of a common mutation , delta F508 , in the CFTR gene allowed , for the first time , the detection of cystic fibrosis ( CF ) carriers in the general population .
	manualset3
155981	6	410395	13	NULL	NULL	0	NULL	detection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of a common mutation , delta F508 , in the CFTR gene allowed , for the first time , the detection of cystic fibrosis ( CF ) carriers in the general population .
	manualset3
155982	7	410395	13	NULL	NULL	0	NULL	cystic fibrosis ( CF ) carriers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of a common mutation , delta F508 , in the CFTR gene allowed , for the first time , the detection of cystic fibrosis ( CF ) carriers in the general population .
	manualset3
155983	8	410395	13	NULL	NULL	0	NULL	general population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of a common mutation , delta F508 , in the CFTR gene allowed , for the first time , the detection of cystic fibrosis ( CF ) carriers in the general population .
	manualset3
155984	1	410396	13	NULL	NULL	0	NULL	identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of a rat VR1 5 ' splice variant and the rat stretch inhibitable channel , which are also expressed in dorsal root ganglia and CNS , raises the possibility that these and/or other VR1 variants may regulate VR1 activity .
	manualset3
155985	2	410396	13	NULL	NULL	0	NULL	 rat VR1 5 ' splice variant 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of a rat VR1 5 ' splice variant and the rat stretch inhibitable channel , which are also expressed in dorsal root ganglia and CNS , raises the possibility that these and/or other VR1 variants may regulate VR1 activity .
	manualset3
155986	3	410396	13	NULL	NULL	0	NULL	rat stretch inhibitable channel 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of a rat VR1 5 ' splice variant and the rat stretch inhibitable channel , which are also expressed in dorsal root ganglia and CNS , raises the possibility that these and/or other VR1 variants may regulate VR1 activity .
	manualset3
155987	4	410396	13	NULL	NULL	0	NULL	 dorsal root ganglia 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of a rat VR1 5 ' splice variant and the rat stretch inhibitable channel , which are also expressed in dorsal root ganglia and CNS , raises the possibility that these and/or other VR1 variants may regulate VR1 activity .
	manualset3
155988	5	410396	13	NULL	NULL	0	NULL	CNS	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of a rat VR1 5 ' splice variant and the rat stretch inhibitable channel , which are also expressed in dorsal root ganglia and CNS , raises the possibility that these and/or other VR1 variants may regulate VR1 activity .
	manualset3
155989	6	410396	13	NULL	NULL	0	NULL	possibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of a rat VR1 5 ' splice variant and the rat stretch inhibitable channel , which are also expressed in dorsal root ganglia and CNS , raises the possibility that these and/or other VR1 variants may regulate VR1 activity .
	manualset3
155990	7	410396	13	NULL	NULL	0	NULL	VR1 variants 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of a rat VR1 5 ' splice variant and the rat stretch inhibitable channel , which are also expressed in dorsal root ganglia and CNS , raises the possibility that these and/or other VR1 variants may regulate VR1 activity .
	manualset3
155991	8	410396	13	NULL	NULL	0	NULL	VR1 activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of a rat VR1 5 ' splice variant and the rat stretch inhibitable channel , which are also expressed in dorsal root ganglia and CNS , raises the possibility that these and/or other VR1 variants may regulate VR1 activity .
	manualset3
155992	1	410397	13	NULL	NULL	0	NULL	identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of additional atopy genes in areas with a certain genetic background is essential for genetic diagnosis and to establish new therapeutic modalities for atopic asthma .
	manualset3
155993	2	410397	13	NULL	NULL	0	NULL	 atopy genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of additional atopy genes in areas with a certain genetic background is essential for genetic diagnosis and to establish new therapeutic modalities for atopic asthma .
	manualset3
155994	3	410397	13	NULL	NULL	0	NULL	areas	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of additional atopy genes in areas with a certain genetic background is essential for genetic diagnosis and to establish new therapeutic modalities for atopic asthma .
	manualset3
155995	4	410397	13	NULL	NULL	0	NULL	genetic background	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of additional atopy genes in areas with a certain genetic background is essential for genetic diagnosis and to establish new therapeutic modalities for atopic asthma .
	manualset3
155996	5	410397	13	NULL	NULL	0	NULL	genetic diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of additional atopy genes in areas with a certain genetic background is essential for genetic diagnosis and to establish new therapeutic modalities for atopic asthma .
	manualset3
155997	6	410397	13	NULL	NULL	0	NULL	therapeutic modalities	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of additional atopy genes in areas with a certain genetic background is essential for genetic diagnosis and to establish new therapeutic modalities for atopic asthma .
	manualset3
155998	7	410397	13	NULL	NULL	0	NULL	atopic asthma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of additional atopy genes in areas with a certain genetic background is essential for genetic diagnosis and to establish new therapeutic modalities for atopic asthma .
	manualset3
155999	1	410398	13	NULL	NULL	0	NULL	identification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of genetic polymorphisms underlying these phenomena does not only explain individual variation in social memory and emotionality , but also help to characterize potential targets for therapeutic interventions .
	manualset3
156000	2	410398	13	NULL	NULL	0	NULL	genetic polymorphisms 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of genetic polymorphisms underlying these phenomena does not only explain individual variation in social memory and emotionality , but also help to characterize potential targets for therapeutic interventions .
	manualset3
156001	3	410398	13	NULL	NULL	0	NULL	phenomena	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of genetic polymorphisms underlying these phenomena does not only explain individual variation in social memory and emotionality , but also help to characterize potential targets for therapeutic interventions .
	manualset3
156002	4	410398	13	NULL	NULL	0	NULL	individual variation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of genetic polymorphisms underlying these phenomena does not only explain individual variation in social memory and emotionality , but also help to characterize potential targets for therapeutic interventions .
	manualset3
156003	5	410398	13	NULL	NULL	0	NULL	social memory	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of genetic polymorphisms underlying these phenomena does not only explain individual variation in social memory and emotionality , but also help to characterize potential targets for therapeutic interventions .
	manualset3
156004	6	410398	13	NULL	NULL	0	NULL	emotionality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of genetic polymorphisms underlying these phenomena does not only explain individual variation in social memory and emotionality , but also help to characterize potential targets for therapeutic interventions .
	manualset3
156005	7	410398	13	NULL	NULL	0	NULL	potential targets 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of genetic polymorphisms underlying these phenomena does not only explain individual variation in social memory and emotionality , but also help to characterize potential targets for therapeutic interventions .
	manualset3
156006	8	410398	13	NULL	NULL	0	NULL	therapeutic interventions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of genetic polymorphisms underlying these phenomena does not only explain individual variation in social memory and emotionality , but also help to characterize potential targets for therapeutic interventions .
	manualset3
156007	1	410399	13	NULL	NULL	0	NULL	identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of the microcyclamide biosynthetic genes provided an avenue by which to study the regulation of peptide synthesis at the transcriptional level .
	manualset3
156008	2	410399	13	NULL	NULL	0	NULL	 microcyclamide biosynthetic genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of the microcyclamide biosynthetic genes provided an avenue by which to study the regulation of peptide synthesis at the transcriptional level .
	manualset3
156009	3	410399	13	NULL	NULL	0	NULL	avenue	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of the microcyclamide biosynthetic genes provided an avenue by which to study the regulation of peptide synthesis at the transcriptional level .
	manualset3
156010	4	410399	13	NULL	NULL	0	NULL	regulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of the microcyclamide biosynthetic genes provided an avenue by which to study the regulation of peptide synthesis at the transcriptional level .
	manualset3
156011	5	410399	13	NULL	NULL	0	NULL	peptide synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of the microcyclamide biosynthetic genes provided an avenue by which to study the regulation of peptide synthesis at the transcriptional level .
	manualset3
156012	6	410399	13	NULL	NULL	0	NULL	transcriptional level	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of the microcyclamide biosynthetic genes provided an avenue by which to study the regulation of peptide synthesis at the transcriptional level .
	manualset3
156013	1	410400	13	NULL	NULL	0	NULL	tendency	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A tendency existed for TBC to decrease over time .
	manualset3
156014	2	410400	13	NULL	NULL	0	NULL	TBC	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A tendency existed for TBC to decrease over time .
	manualset3
156015	3	410400	13	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	A tendency existed for TBC to decrease over time .
	manualset3
156016	1	410401	13	NULL	NULL	0	NULL	carcinogenicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The identified carcinogenicity of O ( 6 ) - methylguanine ( O ( 6 ) - meG ) is largely caused by its miscoding properties .
	manualset3
156017	2	410401	13	NULL	NULL	0	NULL	O ( 6 ) - methylguanine ( O ( 6 ) - meG ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The identified carcinogenicity of O ( 6 ) - methylguanine ( O ( 6 ) - meG ) is largely caused by its miscoding properties .
	manualset3
156018	3	410401	13	NULL	NULL	0	NULL	properties 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The identified carcinogenicity of O ( 6 ) - methylguanine ( O ( 6 ) - meG ) is largely caused by its miscoding properties .
	manualset3
156019	1	410402	13	NULL	NULL	0	NULL	trace residues 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The identified trace residues could provide a reliable and rational guide to the design of CYP51 mutations and give more information about the detailed mechanism of substrate ( drug ) recognition and binding .
	manualset3
156020	2	410402	13	NULL	NULL	0	NULL	rational guide	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The identified trace residues could provide a reliable and rational guide to the design of CYP51 mutations and give more information about the detailed mechanism of substrate ( drug ) recognition and binding .
	manualset3
156021	3	410402	13	NULL	NULL	0	NULL	design	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The identified trace residues could provide a reliable and rational guide to the design of CYP51 mutations and give more information about the detailed mechanism of substrate ( drug ) recognition and binding .
	manualset3
156022	4	410402	13	NULL	NULL	0	NULL	CYP51 mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The identified trace residues could provide a reliable and rational guide to the design of CYP51 mutations and give more information about the detailed mechanism of substrate ( drug ) recognition and binding .
	manualset3
156023	5	410402	13	NULL	NULL	0	NULL	information	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The identified trace residues could provide a reliable and rational guide to the design of CYP51 mutations and give more information about the detailed mechanism of substrate ( drug ) recognition and binding .
	manualset3
156024	6	410402	13	NULL	NULL	0	NULL	mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The identified trace residues could provide a reliable and rational guide to the design of CYP51 mutations and give more information about the detailed mechanism of substrate ( drug ) recognition and binding .
	manualset3
156025	7	410402	13	NULL	NULL	0	NULL	substrate	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The identified trace residues could provide a reliable and rational guide to the design of CYP51 mutations and give more information about the detailed mechanism of substrate ( drug ) recognition and binding .
	manualset3
156026	8	410402	13	NULL	NULL	0	NULL	drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The identified trace residues could provide a reliable and rational guide to the design of CYP51 mutations and give more information about the detailed mechanism of substrate ( drug ) recognition and binding .
	manualset3
156027	9	410402	13	NULL	NULL	0	NULL	 recognition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The identified trace residues could provide a reliable and rational guide to the design of CYP51 mutations and give more information about the detailed mechanism of substrate ( drug ) recognition and binding .
	manualset3
156028	10	410402	13	NULL	NULL	0	NULL	binding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The identified trace residues could provide a reliable and rational guide to the design of CYP51 mutations and give more information about the detailed mechanism of substrate ( drug ) recognition and binding .
	manualset3
156029	1	410403	13	NULL	NULL	0	NULL	 identity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The identity of P37 , stacked between P26 and W68 , was not important for the maintenance of the hydrophobic pocket or for the stability of the complex .
	manualset3
156030	2	410403	13	NULL	NULL	0	NULL	P37 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The identity of P37 , stacked between P26 and W68 , was not important for the maintenance of the hydrophobic pocket or for the stability of the complex .
	manualset3
156031	3	410403	13	NULL	NULL	0	NULL	P26 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The identity of P37 , stacked between P26 and W68 , was not important for the maintenance of the hydrophobic pocket or for the stability of the complex .
	manualset3
156032	4	410403	13	NULL	NULL	0	NULL	W68	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The identity of P37 , stacked between P26 and W68 , was not important for the maintenance of the hydrophobic pocket or for the stability of the complex .
	manualset3
156033	5	410403	13	NULL	NULL	0	NULL	maintenance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The identity of P37 , stacked between P26 and W68 , was not important for the maintenance of the hydrophobic pocket or for the stability of the complex .
	manualset3
156034	6	410403	13	NULL	NULL	0	NULL	hydrophobic pocket 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The identity of P37 , stacked between P26 and W68 , was not important for the maintenance of the hydrophobic pocket or for the stability of the complex .
	manualset3
156035	7	410403	13	NULL	NULL	0	NULL	complex 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The identity of P37 , stacked between P26 and W68 , was not important for the maintenance of the hydrophobic pocket or for the stability of the complex .
	manualset3
156036	1	410404	13	NULL	NULL	0	NULL	 identity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The identity of the cDNA for HMG-CoA synthase was confirmed through comparison of the NH2-terminal amino acid sequence predicted from the cDNA with that determined chemically from the purified enzyme .
	manualset3
156037	2	410404	13	NULL	NULL	0	NULL	 cDNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The identity of the cDNA for HMG-CoA synthase was confirmed through comparison of the NH2-terminal amino acid sequence predicted from the cDNA with that determined chemically from the purified enzyme .
	manualset3
156038	3	410404	13	NULL	NULL	0	NULL	HMG-CoA synthase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The identity of the cDNA for HMG-CoA synthase was confirmed through comparison of the NH2-terminal amino acid sequence predicted from the cDNA with that determined chemically from the purified enzyme .
	manualset3
156039	4	410404	13	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The identity of the cDNA for HMG-CoA synthase was confirmed through comparison of the NH2-terminal amino acid sequence predicted from the cDNA with that determined chemically from the purified enzyme .
	manualset3
156040	5	410404	13	NULL	NULL	0	NULL	NH2-terminal amino acid sequence	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The identity of the cDNA for HMG-CoA synthase was confirmed through comparison of the NH2-terminal amino acid sequence predicted from the cDNA with that determined chemically from the purified enzyme .
	manualset3
156041	6	410404	13	NULL	NULL	0	NULL	cDNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The identity of the cDNA for HMG-CoA synthase was confirmed through comparison of the NH2-terminal amino acid sequence predicted from the cDNA with that determined chemically from the purified enzyme .
	manualset3
156042	7	410404	13	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The identity of the cDNA for HMG-CoA synthase was confirmed through comparison of the NH2-terminal amino acid sequence predicted from the cDNA with that determined chemically from the purified enzyme .
	manualset3
156043	1	410405	13	NULL	NULL	0	NULL	identity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The identity of the thebaine was confirmed by isolation and examination of spectral evidence .
	manualset3
156044	2	410405	13	NULL	NULL	0	NULL	thebaine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The identity of the thebaine was confirmed by isolation and examination of spectral evidence .
	manualset3
156045	3	410405	13	NULL	NULL	0	NULL	isolation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The identity of the thebaine was confirmed by isolation and examination of spectral evidence .
	manualset3
156046	4	410405	13	NULL	NULL	0	NULL	examination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The identity of the thebaine was confirmed by isolation and examination of spectral evidence .
	manualset3
156047	5	410405	13	NULL	NULL	0	NULL	spectral evidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The identity of the thebaine was confirmed by isolation and examination of spectral evidence .
	manualset3
156048	1	410406	13	NULL	NULL	0	NULL	idiosyncratic reactions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The idiosyncratic reactions to the intravenous agents include anaphylactoid reactions ( which are rare ) and triggering of acute porphyria .
	manualset3
156049	2	410406	13	NULL	NULL	0	NULL	intravenous agents	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The idiosyncratic reactions to the intravenous agents include anaphylactoid reactions ( which are rare ) and triggering of acute porphyria .
	manualset3
156050	3	410406	13	NULL	NULL	0	NULL	anaphylactoid reactions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The idiosyncratic reactions to the intravenous agents include anaphylactoid reactions ( which are rare ) and triggering of acute porphyria .
	manualset3
156051	4	410406	13	NULL	NULL	0	NULL	acute porphyria	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The idiosyncratic reactions to the intravenous agents include anaphylactoid reactions ( which are rare ) and triggering of acute porphyria .
	manualset3
157265	5	410406	13	NULL	NULL	0	NULL	triggering	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The idiosyncratic reactions to the intravenous agents include anaphylactoid reactions ( which are rare ) and triggering of acute porphyria .
	manualset3
156052	1	410407	13	NULL	NULL	0	NULL	imNTS	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The imNTS contained oval or ellipsoid-shaped , small to medium-sized neurons ( 18.2 x 11.4 microm ) with little cytoplasm , few cell organelles and an irregularly shaped nucleus .
	manualset3
156053	2	410407	13	NULL	NULL	0	NULL	neurons 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The imNTS contained oval or ellipsoid-shaped , small to medium-sized neurons ( 18.2 x 11.4 microm ) with little cytoplasm , few cell organelles and an irregularly shaped nucleus .
	manualset3
156054	3	410407	13	NULL	NULL	0	NULL	18.2 x 11.4 microm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The imNTS contained oval or ellipsoid-shaped , small to medium-sized neurons ( 18.2 x 11.4 microm ) with little cytoplasm , few cell organelles and an irregularly shaped nucleus .
	manualset3
156055	4	410407	13	NULL	NULL	0	NULL	 cytoplasm	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The imNTS contained oval or ellipsoid-shaped , small to medium-sized neurons ( 18.2 x 11.4 microm ) with little cytoplasm , few cell organelles and an irregularly shaped nucleus .
	manualset3
156056	5	410407	13	NULL	NULL	0	NULL	cell organelles 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The imNTS contained oval or ellipsoid-shaped , small to medium-sized neurons ( 18.2 x 11.4 microm ) with little cytoplasm , few cell organelles and an irregularly shaped nucleus .
	manualset3
156057	6	410407	13	NULL	NULL	0	NULL	nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The imNTS contained oval or ellipsoid-shaped , small to medium-sized neurons ( 18.2 x 11.4 microm ) with little cytoplasm , few cell organelles and an irregularly shaped nucleus .
	manualset3
156058	1	410408	13	NULL	NULL	0	NULL	image quality	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The image quality was clearly superior and the fractional utilization rates of ( 18F ) FDG were twice as high during insulin clamp than after glucose loading ( p less than 0.0001 ) .
	manualset3
156059	2	410408	13	NULL	NULL	0	NULL	 fractional utilization rates	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The image quality was clearly superior and the fractional utilization rates of ( 18F ) FDG were twice as high during insulin clamp than after glucose loading ( p less than 0.0001 ) .
	manualset3
156060	3	410408	13	NULL	NULL	NULL	NULL	 ( 18F ) FDG	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The image quality was clearly superior and the fractional utilization rates of ( 18F ) FDG were twice as high during insulin clamp than after glucose loading ( p less than 0.0001 ) .
	manualset3
156061	4	410408	13	NULL	NULL	0	NULL	insulin clamp	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The image quality was clearly superior and the fractional utilization rates of ( 18F ) FDG were twice as high during insulin clamp than after glucose loading ( p less than 0.0001 ) .
	manualset3
156063	5	410408	13	NULL	NULL	0	NULL	glucose loading 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The image quality was clearly superior and the fractional utilization rates of ( 18F ) FDG were twice as high during insulin clamp than after glucose loading ( p less than 0.0001 ) .
	manualset3
156064	6	410408	13	NULL	NULL	0	NULL	p less than 0.0001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The image quality was clearly superior and the fractional utilization rates of ( 18F ) FDG were twice as high during insulin clamp than after glucose loading ( p less than 0.0001 ) .
	manualset3
156066	1	410409	13	NULL	NULL	0	NULL	imidazole derivative 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The imidazole derivative adsorbs strongly on the surfaces of nanosemiconductor , the apparent binding constants for the association between nanomaterials and imidazole derivative have been determined from the fluorescence quenching .
	manualset3
156067	2	410409	13	NULL	NULL	0	NULL	surfaces of nanosemiconductor	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The imidazole derivative adsorbs strongly on the surfaces of nanosemiconductor , the apparent binding constants for the association between nanomaterials and imidazole derivative have been determined from the fluorescence quenching .
	manualset3
156068	3	410409	13	NULL	NULL	0	NULL	binding constants	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The imidazole derivative adsorbs strongly on the surfaces of nanosemiconductor , the apparent binding constants for the association between nanomaterials and imidazole derivative have been determined from the fluorescence quenching .
	manualset3
156069	4	410409	13	NULL	NULL	0	NULL	association 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The imidazole derivative adsorbs strongly on the surfaces of nanosemiconductor , the apparent binding constants for the association between nanomaterials and imidazole derivative have been determined from the fluorescence quenching .
	manualset3
156070	5	410409	13	NULL	NULL	0	NULL	nanomaterials	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The imidazole derivative adsorbs strongly on the surfaces of nanosemiconductor , the apparent binding constants for the association between nanomaterials and imidazole derivative have been determined from the fluorescence quenching .
	manualset3
156071	6	410409	13	NULL	NULL	0	NULL	imidazole derivative 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The imidazole derivative adsorbs strongly on the surfaces of nanosemiconductor , the apparent binding constants for the association between nanomaterials and imidazole derivative have been determined from the fluorescence quenching .
	manualset3
156072	7	410409	13	NULL	NULL	0	NULL	fluorescence quenching	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The imidazole derivative adsorbs strongly on the surfaces of nanosemiconductor , the apparent binding constants for the association between nanomaterials and imidazole derivative have been determined from the fluorescence quenching .
	manualset3
156075	1	410410	13	NULL	NULL	0	NULL	nondestructive visual analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The immediate nondestructive visual analysis of EGFP expression helps to predict the quality of the viral vector supernatant while it is produced .
	manualset3
156076	2	410410	13	NULL	NULL	0	NULL	EGFP expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The immediate nondestructive visual analysis of EGFP expression helps to predict the quality of the viral vector supernatant while it is produced .
	manualset3
156077	3	410410	13	NULL	NULL	0	NULL	quality 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The immediate nondestructive visual analysis of EGFP expression helps to predict the quality of the viral vector supernatant while it is produced .
	manualset3
156079	4	410410	13	NULL	NULL	0	NULL	viral vector	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The immediate nondestructive visual analysis of EGFP expression helps to predict the quality of the viral vector supernatant while it is produced .
	manualset3
156081	1	410411	13	NULL	NULL	0	NULL	immunological characterization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunological characterization by assessing the cell surface phenotypic markers with monoclonal antibodies and transmission electron microscopy ( TEM ) investigations were also carried out .
	manualset3
156082	2	410411	13	NULL	NULL	NULL	NULL	cell surface phenotypic markers 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The immunological characterization by assessing the cell surface phenotypic markers with monoclonal antibodies and transmission electron microscopy ( TEM ) investigations were also carried out .
	manualset3
156083	3	410411	13	NULL	NULL	0	NULL	monoclonal antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunological characterization by assessing the cell surface phenotypic markers with monoclonal antibodies and transmission electron microscopy ( TEM ) investigations were also carried out .
	manualset3
156084	4	410411	13	NULL	NULL	0	NULL	transmission electron microscopy ( TEM ) investigations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunological characterization by assessing the cell surface phenotypic markers with monoclonal antibodies and transmission electron microscopy ( TEM ) investigations were also carried out .
	manualset3
156085	1	410412	13	NULL	NULL	0	NULL	 effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunomodulating effects of free fucose on intestinal epithelial cells ( enterocyte-like Caco-2 ) were investigated .
	manualset3
156086	2	410412	13	NULL	NULL	0	NULL	 fucose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunomodulating effects of free fucose on intestinal epithelial cells ( enterocyte-like Caco-2 ) were investigated .
	manualset3
156087	3	410412	13	NULL	NULL	0	NULL	 intestinal epithelial cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunomodulating effects of free fucose on intestinal epithelial cells ( enterocyte-like Caco-2 ) were investigated .
	manualset3
156088	4	410412	13	NULL	NULL	0	NULL	enterocyte-like Caco-2	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunomodulating effects of free fucose on intestinal epithelial cells ( enterocyte-like Caco-2 ) were investigated .
	manualset3
156089	1	410413	13	NULL	NULL	0	NULL	immunophenotype	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunophenotype of ovarian stroma and spindle cell tumors derived from ovarian stroma has not been well studied .
	manualset3
156090	2	410413	13	NULL	NULL	0	NULL	ovarian stroma tumors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunophenotype of ovarian stroma and spindle cell tumors derived from ovarian stroma has not been well studied .
	manualset3
156091	3	410413	13	NULL	NULL	0	NULL	ovarian spindle cell tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunophenotype of ovarian stroma and spindle cell tumors derived from ovarian stroma has not been well studied .
	manualset3
156092	4	410413	13	NULL	NULL	0	NULL	ovarian stroma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunophenotype of ovarian stroma and spindle cell tumors derived from ovarian stroma has not been well studied .
	manualset3
156093	1	410414	13	NULL	NULL	0	NULL	immunoprecipitation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunoprecipitation of newly synthesized protein by monospecific antibody raised against pure rat fibrinogen clearly demonstrates that L-epinephrine increased fibrinogen formation in vivo under the experimental condition .
	manualset3
156094	2	410414	13	NULL	NULL	0	NULL	protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunoprecipitation of newly synthesized protein by monospecific antibody raised against pure rat fibrinogen clearly demonstrates that L-epinephrine increased fibrinogen formation in vivo under the experimental condition .
	manualset3
156096	3	410414	13	NULL	NULL	0	NULL	monospecific antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunoprecipitation of newly synthesized protein by monospecific antibody raised against pure rat fibrinogen clearly demonstrates that L-epinephrine increased fibrinogen formation in vivo under the experimental condition .
	manualset3
156097	4	410414	13	NULL	NULL	0	NULL	 pure rat fibrinogen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunoprecipitation of newly synthesized protein by monospecific antibody raised against pure rat fibrinogen clearly demonstrates that L-epinephrine increased fibrinogen formation in vivo under the experimental condition .
	manualset3
156098	5	410414	13	NULL	NULL	0	NULL	L-epinephrine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunoprecipitation of newly synthesized protein by monospecific antibody raised against pure rat fibrinogen clearly demonstrates that L-epinephrine increased fibrinogen formation in vivo under the experimental condition .
	manualset3
156099	6	410414	13	NULL	NULL	0	NULL	fibrinogen formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunoprecipitation of newly synthesized protein by monospecific antibody raised against pure rat fibrinogen clearly demonstrates that L-epinephrine increased fibrinogen formation in vivo under the experimental condition .
	manualset3
156100	7	410414	13	NULL	NULL	0	NULL	experimental condition 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunoprecipitation of newly synthesized protein by monospecific antibody raised against pure rat fibrinogen clearly demonstrates that L-epinephrine increased fibrinogen formation in vivo under the experimental condition .
	manualset3
156102	1	410415	13	NULL	NULL	0	NULL	immunoreactivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunoreactivity was seen in the enlarged basal cells and was seen to focally extend to involve the lumenal cell layer .
	manualset3
156103	2	410415	13	NULL	NULL	0	NULL	basal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunoreactivity was seen in the enlarged basal cells and was seen to focally extend to involve the lumenal cell layer .
	manualset3
156104	3	410415	13	NULL	NULL	0	NULL	lumenal cell layer	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunoreactivity was seen in the enlarged basal cells and was seen to focally extend to involve the lumenal cell layer .
	manualset3
156106	1	410416	13	NULL	NULL	0	NULL	theoretical approach	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A theoretical approach designed for chemical reactions in the condensed phase is used to determine the energy along the reaction path of the enzyme triosephosphate isomerase .
	manualset3
156107	2	410416	13	NULL	NULL	0	NULL	chemical reactions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A theoretical approach designed for chemical reactions in the condensed phase is used to determine the energy along the reaction path of the enzyme triosephosphate isomerase .
	manualset3
156110	3	410416	13	NULL	NULL	0	NULL	condensed phase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A theoretical approach designed for chemical reactions in the condensed phase is used to determine the energy along the reaction path of the enzyme triosephosphate isomerase .
	manualset3
156111	4	410416	13	NULL	NULL	0	NULL	energy 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A theoretical approach designed for chemical reactions in the condensed phase is used to determine the energy along the reaction path of the enzyme triosephosphate isomerase .
	manualset3
156112	5	410416	13	NULL	NULL	0	NULL	reaction path 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A theoretical approach designed for chemical reactions in the condensed phase is used to determine the energy along the reaction path of the enzyme triosephosphate isomerase .
	manualset3
156114	6	410416	13	NULL	NULL	0	NULL	enzyme triosephosphate isomerase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A theoretical approach designed for chemical reactions in the condensed phase is used to determine the energy along the reaction path of the enzyme triosephosphate isomerase .
	manualset3
156116	1	410417	13	NULL	NULL	0	NULL	impact 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of FDG-PET in the management of patients with salivary gland malignancy .
	manualset3
156117	2	410417	13	NULL	NULL	0	NULL	FDG-PET	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of FDG-PET in the management of patients with salivary gland malignancy .
	manualset3
156118	3	410417	13	NULL	NULL	0	NULL	 management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of FDG-PET in the management of patients with salivary gland malignancy .
	manualset3
156119	4	410417	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of FDG-PET in the management of patients with salivary gland malignancy .
	manualset3
156120	5	410417	13	NULL	NULL	0	NULL	salivary gland malignancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of FDG-PET in the management of patients with salivary gland malignancy .
	manualset3
156122	1	410418	13	NULL	NULL	0	NULL	 impact 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of H. avenae on spring wheat yield in the Pacific Northwest had been observed but not quantified .
	manualset3
156123	2	410418	13	NULL	NULL	0	NULL	H. avenae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of H. avenae on spring wheat yield in the Pacific Northwest had been observed but not quantified .
	manualset3
156124	3	410418	13	NULL	NULL	0	NULL	spring wheat yield	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of H. avenae on spring wheat yield in the Pacific Northwest had been observed but not quantified .
	manualset3
156125	4	410418	13	NULL	NULL	0	NULL	Pacific Northwest 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of H. avenae on spring wheat yield in the Pacific Northwest had been observed but not quantified .
	manualset3
156127	1	410419	13	NULL	NULL	0	NULL	impact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of brewing yeast cell age on fermentation performance , attenuation and flocculation .
	manualset3
156128	2	410419	13	NULL	NULL	0	NULL	yeast cell age 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of brewing yeast cell age on fermentation performance , attenuation and flocculation .
	manualset3
156129	3	410419	13	NULL	NULL	0	NULL	fermentation performance	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of brewing yeast cell age on fermentation performance , attenuation and flocculation .
	manualset3
156131	4	410419	13	NULL	NULL	0	NULL	attenuation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of brewing yeast cell age on fermentation performance , attenuation and flocculation .
	manualset3
156132	5	410419	13	NULL	NULL	0	NULL	flocculation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of brewing yeast cell age on fermentation performance , attenuation and flocculation .
	manualset3
156133	1	410420	13	NULL	NULL	0	NULL	 impact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of crime on urban women .
	manualset3
156134	2	410420	13	NULL	NULL	0	NULL	 crime	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of crime on urban women .
	manualset3
156135	3	410420	13	NULL	NULL	0	NULL	urban women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of crime on urban women .
	manualset3
156136	1	410421	13	NULL	NULL	0	NULL	impact	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of the gsp oncogene on the expression of genes engaged in the somatotroph cell phenotype remains poorly understood in human somatotroph adenomas .
	manualset3
156137	2	410421	13	NULL	NULL	0	NULL	 gsp oncogene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of the gsp oncogene on the expression of genes engaged in the somatotroph cell phenotype remains poorly understood in human somatotroph adenomas .
	manualset3
156138	3	410421	13	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of the gsp oncogene on the expression of genes engaged in the somatotroph cell phenotype remains poorly understood in human somatotroph adenomas .
	manualset3
156139	4	410421	13	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of the gsp oncogene on the expression of genes engaged in the somatotroph cell phenotype remains poorly understood in human somatotroph adenomas .
	manualset3
156140	5	410421	13	NULL	NULL	0	NULL	somatotroph cell phenotype	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of the gsp oncogene on the expression of genes engaged in the somatotroph cell phenotype remains poorly understood in human somatotroph adenomas .
	manualset3
156141	6	410421	13	NULL	NULL	0	NULL	human somatotroph adenomas 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of the gsp oncogene on the expression of genes engaged in the somatotroph cell phenotype remains poorly understood in human somatotroph adenomas .
	manualset3
156143	1	410422	13	NULL	NULL	0	NULL	 impact 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of three organic acid producing fungi ( Aspergillus niger , Serpula himantioides and Trametes versicolor ) on apatite , galena and obsidian was examined in the absence and presence of a carbon and energy source ( glucose ) .
	manualset3
156144	2	410422	13	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of three organic acid producing fungi ( Aspergillus niger , Serpula himantioides and Trametes versicolor ) on apatite , galena and obsidian was examined in the absence and presence of a carbon and energy source ( glucose ) .
	manualset3
156145	3	410422	13	NULL	NULL	0	NULL	organic acid producing fungi 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of three organic acid producing fungi ( Aspergillus niger , Serpula himantioides and Trametes versicolor ) on apatite , galena and obsidian was examined in the absence and presence of a carbon and energy source ( glucose ) .
	manualset3
156146	4	410422	13	NULL	NULL	0	NULL	Aspergillus niger 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of three organic acid producing fungi ( Aspergillus niger , Serpula himantioides and Trametes versicolor ) on apatite , galena and obsidian was examined in the absence and presence of a carbon and energy source ( glucose ) .
	manualset3
156147	5	410422	13	NULL	NULL	0	NULL	Serpula himantioides	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of three organic acid producing fungi ( Aspergillus niger , Serpula himantioides and Trametes versicolor ) on apatite , galena and obsidian was examined in the absence and presence of a carbon and energy source ( glucose ) .
	manualset3
156148	6	410422	13	NULL	NULL	0	NULL	Trametes versicolor	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of three organic acid producing fungi ( Aspergillus niger , Serpula himantioides and Trametes versicolor ) on apatite , galena and obsidian was examined in the absence and presence of a carbon and energy source ( glucose ) .
	manualset3
156149	7	410422	13	NULL	NULL	0	NULL	apatite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of three organic acid producing fungi ( Aspergillus niger , Serpula himantioides and Trametes versicolor ) on apatite , galena and obsidian was examined in the absence and presence of a carbon and energy source ( glucose ) .
	manualset3
156150	8	410422	13	NULL	NULL	0	NULL	galena	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of three organic acid producing fungi ( Aspergillus niger , Serpula himantioides and Trametes versicolor ) on apatite , galena and obsidian was examined in the absence and presence of a carbon and energy source ( glucose ) .
	manualset3
156151	9	410422	13	NULL	NULL	0	NULL	obsidian 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of three organic acid producing fungi ( Aspergillus niger , Serpula himantioides and Trametes versicolor ) on apatite , galena and obsidian was examined in the absence and presence of a carbon and energy source ( glucose ) .
	manualset3
156152	10	410422	13	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of three organic acid producing fungi ( Aspergillus niger , Serpula himantioides and Trametes versicolor ) on apatite , galena and obsidian was examined in the absence and presence of a carbon and energy source ( glucose ) .
	manualset3
156153	11	410422	13	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of three organic acid producing fungi ( Aspergillus niger , Serpula himantioides and Trametes versicolor ) on apatite , galena and obsidian was examined in the absence and presence of a carbon and energy source ( glucose ) .
	manualset3
156154	12	410422	13	NULL	NULL	0	NULL	carbon and energy source	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of three organic acid producing fungi ( Aspergillus niger , Serpula himantioides and Trametes versicolor ) on apatite , galena and obsidian was examined in the absence and presence of a carbon and energy source ( glucose ) .
	manualset3
156155	13	410422	13	NULL	NULL	0	NULL	glucose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The impact of three organic acid producing fungi ( Aspergillus niger , Serpula himantioides and Trametes versicolor ) on apatite , galena and obsidian was examined in the absence and presence of a carbon and energy source ( glucose ) .
	manualset3
156162	1	410423	13	NULL	NULL	0	NULL	implantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The implantation of an SCS system is a surgical procedure , which requires the highest standards in asepsis .
	manualset3
156163	2	410423	13	NULL	NULL	0	NULL	SCS system	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The implantation of an SCS system is a surgical procedure , which requires the highest standards in asepsis .
	manualset3
156165	3	410423	13	NULL	NULL	0	NULL	surgical procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The implantation of an SCS system is a surgical procedure , which requires the highest standards in asepsis .
	manualset3
156166	4	410423	13	NULL	NULL	0	NULL	standards	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The implantation of an SCS system is a surgical procedure , which requires the highest standards in asepsis .
	manualset3
156167	5	410423	13	NULL	NULL	0	NULL	asepsis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The implantation of an SCS system is a surgical procedure , which requires the highest standards in asepsis .
	manualset3
156168	1	410424	13	NULL	NULL	0	NULL	implantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The implantation of the pancreatic tissues with hypothalamic neuropeptidergic ( supra optic ) nuclei was also performed using light and electron microscopy and histochemistry .
	manualset3
156169	2	410424	13	NULL	NULL	0	NULL	pancreatic tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The implantation of the pancreatic tissues with hypothalamic neuropeptidergic ( supra optic ) nuclei was also performed using light and electron microscopy and histochemistry .
	manualset3
156170	3	410424	13	NULL	NULL	0	NULL	hypothalamic neuropeptidergic ( supra optic ) nuclei	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The implantation of the pancreatic tissues with hypothalamic neuropeptidergic ( supra optic ) nuclei was also performed using light and electron microscopy and histochemistry .
	manualset3
156171	4	410424	13	NULL	NULL	0	NULL	light microscopy 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The implantation of the pancreatic tissues with hypothalamic neuropeptidergic ( supra optic ) nuclei was also performed using light and electron microscopy and histochemistry .
	manualset3
156172	5	410424	13	NULL	NULL	0	NULL	electron microscopy	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The implantation of the pancreatic tissues with hypothalamic neuropeptidergic ( supra optic ) nuclei was also performed using light and electron microscopy and histochemistry .
	manualset3
156173	6	410424	13	NULL	NULL	0	NULL	histochemistry	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The implantation of the pancreatic tissues with hypothalamic neuropeptidergic ( supra optic ) nuclei was also performed using light and electron microscopy and histochemistry .
	manualset3
156174	1	410425	13	NULL	NULL	0	NULL	implications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications of symptom validity test failure for ability-based test performance in a pediatric sample .
	manualset3
156175	2	410425	13	NULL	NULL	0	NULL	symptom validity test failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications of symptom validity test failure for ability-based test performance in a pediatric sample .
	manualset3
156176	3	410425	13	NULL	NULL	NULL	NULL	ability-based test performance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The implications of symptom validity test failure for ability-based test performance in a pediatric sample .
	manualset3
156177	4	410425	13	NULL	NULL	NULL	NULL	pediatric sample	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The implications of symptom validity test failure for ability-based test performance in a pediatric sample .
	manualset3
156179	1	410426	13	NULL	NULL	0	NULL	implications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications of these findings are discussed in terms of the active moiety responsible for the primary action of HC-3 on ACh synthesis .
	manualset3
156180	2	410426	13	NULL	NULL	0	NULL	findings	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications of these findings are discussed in terms of the active moiety responsible for the primary action of HC-3 on ACh synthesis .
	manualset3
156181	3	410426	13	NULL	NULL	0	NULL	terms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications of these findings are discussed in terms of the active moiety responsible for the primary action of HC-3 on ACh synthesis .
	manualset3
156182	4	410426	13	NULL	NULL	0	NULL	active moiety	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications of these findings are discussed in terms of the active moiety responsible for the primary action of HC-3 on ACh synthesis .
	manualset3
156183	5	410426	13	NULL	NULL	0	NULL	primary action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications of these findings are discussed in terms of the active moiety responsible for the primary action of HC-3 on ACh synthesis .
	manualset3
156185	6	410426	13	NULL	NULL	0	NULL	HC-3	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications of these findings are discussed in terms of the active moiety responsible for the primary action of HC-3 on ACh synthesis .
	manualset3
156186	7	410426	13	NULL	NULL	0	NULL	ACh synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications of these findings are discussed in terms of the active moiety responsible for the primary action of HC-3 on ACh synthesis .
	manualset3
156191	1	410427	13	NULL	NULL	0	NULL	implications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications of these findings for adaptation to protein restriction and a discussion of equilibrium and steady state conditions related to the increase in methionine content in the blood are presented .
	manualset3
156192	2	410427	13	NULL	NULL	0	NULL	findings 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications of these findings for adaptation to protein restriction and a discussion of equilibrium and steady state conditions related to the increase in methionine content in the blood are presented .
	manualset3
156194	3	410427	13	NULL	NULL	0	NULL	adaptation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications of these findings for adaptation to protein restriction and a discussion of equilibrium and steady state conditions related to the increase in methionine content in the blood are presented .
	manualset3
156195	4	410427	13	NULL	NULL	0	NULL	protein restriction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications of these findings for adaptation to protein restriction and a discussion of equilibrium and steady state conditions related to the increase in methionine content in the blood are presented .
	manualset3
156196	5	410427	13	NULL	NULL	0	NULL	discussion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications of these findings for adaptation to protein restriction and a discussion of equilibrium and steady state conditions related to the increase in methionine content in the blood are presented .
	manualset3
156197	6	410427	13	NULL	NULL	0	NULL	equilibrium conditions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications of these findings for adaptation to protein restriction and a discussion of equilibrium and steady state conditions related to the increase in methionine content in the blood are presented .
	manualset3
156198	7	410427	13	NULL	NULL	0	NULL	steady state conditions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications of these findings for adaptation to protein restriction and a discussion of equilibrium and steady state conditions related to the increase in methionine content in the blood are presented .
	manualset3
156199	8	410427	13	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications of these findings for adaptation to protein restriction and a discussion of equilibrium and steady state conditions related to the increase in methionine content in the blood are presented .
	manualset3
156200	9	410427	13	NULL	NULL	0	NULL	methionine content	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications of these findings for adaptation to protein restriction and a discussion of equilibrium and steady state conditions related to the increase in methionine content in the blood are presented .
	manualset3
156201	10	410427	13	NULL	NULL	0	NULL	blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications of these findings for adaptation to protein restriction and a discussion of equilibrium and steady state conditions related to the increase in methionine content in the blood are presented .
	manualset3
156206	1	410428	13	NULL	NULL	0	NULL	biofilm	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	A thick biofilm is formed within 24 hours on the entire surface of these plastic devices once inoculated even with a small initial number of bacteria .
	manualset3
156207	2	410428	13	NULL	NULL	0	NULL	24 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A thick biofilm is formed within 24 hours on the entire surface of these plastic devices once inoculated even with a small initial number of bacteria .
	manualset3
156208	3	410428	13	NULL	NULL	0	NULL	surface 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	A thick biofilm is formed within 24 hours on the entire surface of these plastic devices once inoculated even with a small initial number of bacteria .
	manualset3
156209	4	410428	13	NULL	NULL	0	NULL	plastic devices 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	A thick biofilm is formed within 24 hours on the entire surface of these plastic devices once inoculated even with a small initial number of bacteria .
	manualset3
156210	5	410428	13	NULL	NULL	0	NULL	 small initial number	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A thick biofilm is formed within 24 hours on the entire surface of these plastic devices once inoculated even with a small initial number of bacteria .
	manualset3
156211	6	410428	13	NULL	NULL	0	NULL	bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A thick biofilm is formed within 24 hours on the entire surface of these plastic devices once inoculated even with a small initial number of bacteria .
	manualset3
156212	1	410429	13	NULL	NULL	0	NULL	implications 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications of these observations are discussed in the context of mechanisms of host defense in tuberculosis .
	manualset3
156213	2	410429	13	NULL	NULL	0	NULL	observations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications of these observations are discussed in the context of mechanisms of host defense in tuberculosis .
	manualset3
156214	3	410429	13	NULL	NULL	0	NULL	context	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications of these observations are discussed in the context of mechanisms of host defense in tuberculosis .
	manualset3
156215	4	410429	13	NULL	NULL	0	NULL	mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications of these observations are discussed in the context of mechanisms of host defense in tuberculosis .
	manualset3
156216	5	410429	13	NULL	NULL	0	NULL	 host defense 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications of these observations are discussed in the context of mechanisms of host defense in tuberculosis .
	manualset3
156217	6	410429	13	NULL	NULL	0	NULL	tuberculosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications of these observations are discussed in the context of mechanisms of host defense in tuberculosis .
	manualset3
156219	1	410430	13	NULL	NULL	0	NULL	 importance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The importance of a thorough neuropathological examination in all cases of sudden death , in which no extracerebral cause had been found , is emphasized .
	manualset3
156220	2	410430	13	NULL	NULL	0	NULL	neuropathological examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The importance of a thorough neuropathological examination in all cases of sudden death , in which no extracerebral cause had been found , is emphasized .
	manualset3
156221	3	410430	13	NULL	NULL	0	NULL	cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The importance of a thorough neuropathological examination in all cases of sudden death , in which no extracerebral cause had been found , is emphasized .
	manualset3
156222	4	410430	13	NULL	NULL	0	NULL	death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The importance of a thorough neuropathological examination in all cases of sudden death , in which no extracerebral cause had been found , is emphasized .
	manualset3
156223	5	410430	13	NULL	NULL	0	NULL	cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The importance of a thorough neuropathological examination in all cases of sudden death , in which no extracerebral cause had been found , is emphasized .
	manualset3
168875	1	410431	13	NULL	NULL	0	NULL	importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The importance of drug delivery is pivotal in the wide area of pharmacological research .
	manualset3
168877	3	410431	13	NULL	NULL	NULL	NULL	drug delivery 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The importance of drug delivery is pivotal in the wide area of pharmacological research .
	manualset3
168878	4	410431	13	NULL	NULL	0	NULL	pharmacological research 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The importance of drug delivery is pivotal in the wide area of pharmacological research .
	manualset3
168879	1	410432	13	NULL	NULL	0	NULL	importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The importance of linoleic acid metabolites in cancer metastasis and in the synthesis and actions of 13-HODE .
	manualset3
168880	2	410432	13	NULL	NULL	0	NULL	 linoleic acid metabolites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The importance of linoleic acid metabolites in cancer metastasis and in the synthesis and actions of 13-HODE .
	manualset3
168881	3	410432	13	NULL	NULL	0	NULL	cancer metastasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The importance of linoleic acid metabolites in cancer metastasis and in the synthesis and actions of 13-HODE .
	manualset3
168882	4	410432	13	NULL	NULL	0	NULL	synthesis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The importance of linoleic acid metabolites in cancer metastasis and in the synthesis and actions of 13-HODE .
	manualset3
168883	5	410432	13	NULL	NULL	0	NULL	actions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The importance of linoleic acid metabolites in cancer metastasis and in the synthesis and actions of 13-HODE .
	manualset3
168884	6	410432	13	NULL	NULL	0	NULL	13-HODE	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The importance of linoleic acid metabolites in cancer metastasis and in the synthesis and actions of 13-HODE .
	manualset3
168885	1	410433	13	NULL	NULL	0	NULL	importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The importance of meticulous staging can not be overstated .
	manualset3
168886	2	410433	13	NULL	NULL	0	NULL	meticulous staging	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The importance of meticulous staging can not be overstated .
	manualset3
168889	1	410434	13	NULL	NULL	0	NULL	importance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The importance of skilled management to maintain pasture quality and optimise animal performance under inconsistent climatic conditions should not be underestimated .
	manualset3
168890	2	410434	13	NULL	NULL	0	NULL	management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The importance of skilled management to maintain pasture quality and optimise animal performance under inconsistent climatic conditions should not be underestimated .
	manualset3
168891	3	410434	13	NULL	NULL	0	NULL	pasture quality	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The importance of skilled management to maintain pasture quality and optimise animal performance under inconsistent climatic conditions should not be underestimated .
	manualset3
168892	4	410434	13	NULL	NULL	0	NULL	optimise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The importance of skilled management to maintain pasture quality and optimise animal performance under inconsistent climatic conditions should not be underestimated .
	manualset3
168893	5	410434	13	NULL	NULL	0	NULL	animal performance 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The importance of skilled management to maintain pasture quality and optimise animal performance under inconsistent climatic conditions should not be underestimated .
	manualset3
168894	6	410434	13	NULL	NULL	NULL	NULL	climatic conditions 	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The importance of skilled management to maintain pasture quality and optimise animal performance under inconsistent climatic conditions should not be underestimated .
	manualset3
168898	1	410435	13	NULL	NULL	0	NULL	concept	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The important concept of sterile inflammation is explained against the backdrop of classical inflammation , and its key differences from what researchers refer to when they use the terms neuroinflammation and microglial inflammation are illustrated .
	manualset3
168899	2	410435	13	NULL	NULL	0	NULL	sterile inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The important concept of sterile inflammation is explained against the backdrop of classical inflammation , and its key differences from what researchers refer to when they use the terms neuroinflammation and microglial inflammation are illustrated .
	manualset3
168900	3	410435	13	NULL	NULL	0	NULL	backdrop	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The important concept of sterile inflammation is explained against the backdrop of classical inflammation , and its key differences from what researchers refer to when they use the terms neuroinflammation and microglial inflammation are illustrated .
	manualset3
168901	4	410435	13	NULL	NULL	0	NULL	classical inflammation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The important concept of sterile inflammation is explained against the backdrop of classical inflammation , and its key differences from what researchers refer to when they use the terms neuroinflammation and microglial inflammation are illustrated .
	manualset3
168902	5	410435	13	NULL	NULL	0	NULL	key differences	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The important concept of sterile inflammation is explained against the backdrop of classical inflammation , and its key differences from what researchers refer to when they use the terms neuroinflammation and microglial inflammation are illustrated .
	manualset3
168903	6	410435	13	NULL	NULL	0	NULL	researchers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The important concept of sterile inflammation is explained against the backdrop of classical inflammation , and its key differences from what researchers refer to when they use the terms neuroinflammation and microglial inflammation are illustrated .
	manualset3
168904	7	410435	13	NULL	NULL	0	NULL	terms	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The important concept of sterile inflammation is explained against the backdrop of classical inflammation , and its key differences from what researchers refer to when they use the terms neuroinflammation and microglial inflammation are illustrated .
	manualset3
168905	8	410435	13	NULL	NULL	0	NULL	neuroinflammation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The important concept of sterile inflammation is explained against the backdrop of classical inflammation , and its key differences from what researchers refer to when they use the terms neuroinflammation and microglial inflammation are illustrated .
	manualset3
168906	9	410435	13	NULL	NULL	0	NULL	microglial inflammation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The important concept of sterile inflammation is explained against the backdrop of classical inflammation , and its key differences from what researchers refer to when they use the terms neuroinflammation and microglial inflammation are illustrated .
	manualset3
168907	1	410436	13	NULL	NULL	0	NULL	thiol peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	A thiol peptide , which recently was shown to be a potent inhibitor of corneal collagenase in vitro , was tested in alkali-burned rabbit corneas to determine its effectiveness in inhibiting corneal ulceration .
	manualset3
168908	2	410436	13	NULL	NULL	0	NULL	inhibitor 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	A thiol peptide , which recently was shown to be a potent inhibitor of corneal collagenase in vitro , was tested in alkali-burned rabbit corneas to determine its effectiveness in inhibiting corneal ulceration .
	manualset3
168909	3	410436	13	NULL	NULL	0	NULL	corneal collagenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A thiol peptide , which recently was shown to be a potent inhibitor of corneal collagenase in vitro , was tested in alkali-burned rabbit corneas to determine its effectiveness in inhibiting corneal ulceration .
	manualset3
168910	4	410436	13	NULL	NULL	0	NULL	rabbit corneas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A thiol peptide , which recently was shown to be a potent inhibitor of corneal collagenase in vitro , was tested in alkali-burned rabbit corneas to determine its effectiveness in inhibiting corneal ulceration .
	manualset3
168911	5	410436	13	NULL	NULL	0	NULL	effectiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A thiol peptide , which recently was shown to be a potent inhibitor of corneal collagenase in vitro , was tested in alkali-burned rabbit corneas to determine its effectiveness in inhibiting corneal ulceration .
	manualset3
168912	6	410436	13	NULL	NULL	0	NULL	corneal ulceration 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A thiol peptide , which recently was shown to be a potent inhibitor of corneal collagenase in vitro , was tested in alkali-burned rabbit corneas to determine its effectiveness in inhibiting corneal ulceration .
	manualset3
168913	1	410437	13	NULL	NULL	0	NULL	difference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The important difference between proton and x-ray therapy is in the dose distribution .
	manualset3
168914	2	410437	13	NULL	NULL	0	NULL	proton therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The important difference between proton and x-ray therapy is in the dose distribution .
	manualset3
168915	3	410437	13	NULL	NULL	0	NULL	x-ray therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The important difference between proton and x-ray therapy is in the dose distribution .
	manualset3
168916	4	410437	13	NULL	NULL	0	NULL	dose distribution	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The important difference between proton and x-ray therapy is in the dose distribution .
	manualset3
168917	1	410438	13	NULL	NULL	0	NULL	parameters	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The important parameters in the model were the antigen density entering the lymph node and the propensity of the antigens to induce naive T cells down a specific TH subset pathway .
	manualset3
168918	2	410438	13	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The important parameters in the model were the antigen density entering the lymph node and the propensity of the antigens to induce naive T cells down a specific TH subset pathway .
	manualset3
168919	3	410438	13	NULL	NULL	0	NULL	antigen density	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The important parameters in the model were the antigen density entering the lymph node and the propensity of the antigens to induce naive T cells down a specific TH subset pathway .
	manualset3
168920	4	410438	13	NULL	NULL	NULL	NULL	lymph node	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The important parameters in the model were the antigen density entering the lymph node and the propensity of the antigens to induce naive T cells down a specific TH subset pathway .
	manualset3
168921	5	410438	13	NULL	NULL	0	NULL	propensity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The important parameters in the model were the antigen density entering the lymph node and the propensity of the antigens to induce naive T cells down a specific TH subset pathway .
	manualset3
168922	6	410438	13	NULL	NULL	0	NULL	antigens	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The important parameters in the model were the antigen density entering the lymph node and the propensity of the antigens to induce naive T cells down a specific TH subset pathway .
	manualset3
168923	7	410438	13	NULL	NULL	0	NULL	naive T cells 	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The important parameters in the model were the antigen density entering the lymph node and the propensity of the antigens to induce naive T cells down a specific TH subset pathway .
	manualset3
168924	8	410438	13	NULL	NULL	0	NULL	TH subset pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The important parameters in the model were the antigen density entering the lymph node and the propensity of the antigens to induce naive T cells down a specific TH subset pathway .
	manualset3
168925	1	410439	13	NULL	NULL	0	NULL	role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The important role of immunological ( T cells and Ig ) , infective ( microorganisms and bacterial biofilms ) and allergic factors as predisposing factors for otitis media leads one to consider the importance of a medical treatment oriented to correction of the infective and immunological disorders in children with OM , without adenoids hypertrophy .
	manualset3
168926	2	410439	13	NULL	NULL	0	NULL	immunological T cells 	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The important role of immunological ( T cells and Ig ) , infective ( microorganisms and bacterial biofilms ) and allergic factors as predisposing factors for otitis media leads one to consider the importance of a medical treatment oriented to correction of the infective and immunological disorders in children with OM , without adenoids hypertrophy .
	manualset3
168927	3	410439	13	NULL	NULL	0	NULL	Ig 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The important role of immunological ( T cells and Ig ) , infective ( microorganisms and bacterial biofilms ) and allergic factors as predisposing factors for otitis media leads one to consider the importance of a medical treatment oriented to correction of the infective and immunological disorders in children with OM , without adenoids hypertrophy .
	manualset3
168928	4	410439	13	NULL	NULL	0	NULL	microorganisms 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The important role of immunological ( T cells and Ig ) , infective ( microorganisms and bacterial biofilms ) and allergic factors as predisposing factors for otitis media leads one to consider the importance of a medical treatment oriented to correction of the infective and immunological disorders in children with OM , without adenoids hypertrophy .
	manualset3
168929	5	410439	13	NULL	NULL	NULL	NULL	bacterial biofilms	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The important role of immunological ( T cells and Ig ) , infective ( microorganisms and bacterial biofilms ) and allergic factors as predisposing factors for otitis media leads one to consider the importance of a medical treatment oriented to correction of the infective and immunological disorders in children with OM , without adenoids hypertrophy .
	manualset3
168930	6	410439	13	NULL	NULL	0	NULL	allergic factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The important role of immunological ( T cells and Ig ) , infective ( microorganisms and bacterial biofilms ) and allergic factors as predisposing factors for otitis media leads one to consider the importance of a medical treatment oriented to correction of the infective and immunological disorders in children with OM , without adenoids hypertrophy .
	manualset3
168931	7	410439	13	NULL	NULL	0	NULL	factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The important role of immunological ( T cells and Ig ) , infective ( microorganisms and bacterial biofilms ) and allergic factors as predisposing factors for otitis media leads one to consider the importance of a medical treatment oriented to correction of the infective and immunological disorders in children with OM , without adenoids hypertrophy .
	manualset3
168932	8	410439	13	NULL	NULL	NULL	NULL	otitis media	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The important role of immunological ( T cells and Ig ) , infective ( microorganisms and bacterial biofilms ) and allergic factors as predisposing factors for otitis media leads one to consider the importance of a medical treatment oriented to correction of the infective and immunological disorders in children with OM , without adenoids hypertrophy .
	manualset3
168933	9	410439	13	NULL	NULL	0	NULL	importance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The important role of immunological ( T cells and Ig ) , infective ( microorganisms and bacterial biofilms ) and allergic factors as predisposing factors for otitis media leads one to consider the importance of a medical treatment oriented to correction of the infective and immunological disorders in children with OM , without adenoids hypertrophy .
	manualset3
168934	10	410439	13	NULL	NULL	0	NULL	medical treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The important role of immunological ( T cells and Ig ) , infective ( microorganisms and bacterial biofilms ) and allergic factors as predisposing factors for otitis media leads one to consider the importance of a medical treatment oriented to correction of the infective and immunological disorders in children with OM , without adenoids hypertrophy .
	manualset3
168935	11	410439	13	NULL	NULL	0	NULL	correction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The important role of immunological ( T cells and Ig ) , infective ( microorganisms and bacterial biofilms ) and allergic factors as predisposing factors for otitis media leads one to consider the importance of a medical treatment oriented to correction of the infective and immunological disorders in children with OM , without adenoids hypertrophy .
	manualset3
168936	12	410439	13	NULL	NULL	0	NULL	infective disorders 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The important role of immunological ( T cells and Ig ) , infective ( microorganisms and bacterial biofilms ) and allergic factors as predisposing factors for otitis media leads one to consider the importance of a medical treatment oriented to correction of the infective and immunological disorders in children with OM , without adenoids hypertrophy .
	manualset3
168937	13	410439	13	NULL	NULL	0	NULL	immunological disorders 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The important role of immunological ( T cells and Ig ) , infective ( microorganisms and bacterial biofilms ) and allergic factors as predisposing factors for otitis media leads one to consider the importance of a medical treatment oriented to correction of the infective and immunological disorders in children with OM , without adenoids hypertrophy .
	manualset3
168938	14	410439	13	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The important role of immunological ( T cells and Ig ) , infective ( microorganisms and bacterial biofilms ) and allergic factors as predisposing factors for otitis media leads one to consider the importance of a medical treatment oriented to correction of the infective and immunological disorders in children with OM , without adenoids hypertrophy .
	manualset3
168939	15	410439	13	NULL	NULL	0	NULL	OM	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The important role of immunological ( T cells and Ig ) , infective ( microorganisms and bacterial biofilms ) and allergic factors as predisposing factors for otitis media leads one to consider the importance of a medical treatment oriented to correction of the infective and immunological disorders in children with OM , without adenoids hypertrophy .
	manualset3
168941	16	410439	13	NULL	NULL	0	NULL	adenoids hypertrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The important role of immunological ( T cells and Ig ) , infective ( microorganisms and bacterial biofilms ) and allergic factors as predisposing factors for otitis media leads one to consider the importance of a medical treatment oriented to correction of the infective and immunological disorders in children with OM , without adenoids hypertrophy .
	manualset3
168942	1	410440	13	NULL	NULL	0	NULL	antineoplastic effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The improved antineoplastic effects could be ascribed to its small vesicle size , which allowed more drug release after the accumulation into tumor zone .
	manualset3
168943	2	410440	13	NULL	NULL	0	NULL	small vesicle size	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The improved antineoplastic effects could be ascribed to its small vesicle size , which allowed more drug release after the accumulation into tumor zone .
	manualset3
168944	3	410440	13	NULL	NULL	0	NULL	drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The improved antineoplastic effects could be ascribed to its small vesicle size , which allowed more drug release after the accumulation into tumor zone .
	manualset3
168945	4	410440	13	NULL	NULL	0	NULL	release	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The improved antineoplastic effects could be ascribed to its small vesicle size , which allowed more drug release after the accumulation into tumor zone .
	manualset3
168946	5	410440	13	NULL	NULL	0	NULL	accumulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The improved antineoplastic effects could be ascribed to its small vesicle size , which allowed more drug release after the accumulation into tumor zone .
	manualset3
168947	6	410440	13	NULL	NULL	NULL	NULL	tumor zone	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The improved antineoplastic effects could be ascribed to its small vesicle size , which allowed more drug release after the accumulation into tumor zone .
	manualset3
168948	1	410441	13	NULL	NULL	0	NULL	improvement ratio	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The improvement ratio increased depending on follow-up period : 30.4 % in 6 months , 65.0 % in 1 year , and 67.9 % in 2 years .
	manualset3
168949	2	410441	13	NULL	NULL	0	NULL	follow-up period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The improvement ratio increased depending on follow-up period : 30.4 % in 6 months , 65.0 % in 1 year , and 67.9 % in 2 years .
	manualset3
168950	3	410441	13	NULL	NULL	0	NULL	30.4 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The improvement ratio increased depending on follow-up period : 30.4 % in 6 months , 65.0 % in 1 year , and 67.9 % in 2 years .
	manualset3
168951	4	410441	13	NULL	NULL	0	NULL	6 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The improvement ratio increased depending on follow-up period : 30.4 % in 6 months , 65.0 % in 1 year , and 67.9 % in 2 years .
	manualset3
168952	5	410441	13	NULL	NULL	NULL	NULL	65.0 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The improvement ratio increased depending on follow-up period : 30.4 % in 6 months , 65.0 % in 1 year , and 67.9 % in 2 years .
	manualset3
168955	6	410441	13	NULL	NULL	0	NULL	1 year	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The improvement ratio increased depending on follow-up period : 30.4 % in 6 months , 65.0 % in 1 year , and 67.9 % in 2 years .
	manualset3
168956	7	410441	13	NULL	NULL	0	NULL	67.9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The improvement ratio increased depending on follow-up period : 30.4 % in 6 months , 65.0 % in 1 year , and 67.9 % in 2 years .
	manualset3
168957	8	410441	13	NULL	NULL	0	NULL	2 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The improvement ratio increased depending on follow-up period : 30.4 % in 6 months , 65.0 % in 1 year , and 67.9 % in 2 years .
	manualset3
168958	1	410442	13	NULL	NULL	0	NULL	susceptibility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The in-vitro susceptibility to the cephalosporins differs among strains .
	manualset3
168959	2	410442	13	NULL	NULL	0	NULL	cephalosporins	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The in-vitro susceptibility to the cephalosporins differs among strains .
	manualset3
168960	3	410442	13	NULL	NULL	0	NULL	strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The in-vitro susceptibility to the cephalosporins differs among strains .
	manualset3
168961	1	410443	13	NULL	NULL	0	NULL	32P	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro 32P incorporation into NF-H was also determined .
	manualset3
168962	2	410443	13	NULL	NULL	0	NULL	incorporation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro 32P incorporation into NF-H was also determined .
	manualset3
168963	3	410443	13	NULL	NULL	0	NULL	NF-H	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro 32P incorporation into NF-H was also determined .
	manualset3
168964	1	410444	13	NULL	NULL	0	NULL	activities 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro activities of penicillin and ceftriaxone were compared against 29 strains of Streptococcus pyogenes with the result that ceftriaxone showed greater activity than penicillin .
	manualset3
168965	2	410444	13	NULL	NULL	0	NULL	penicillin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro activities of penicillin and ceftriaxone were compared against 29 strains of Streptococcus pyogenes with the result that ceftriaxone showed greater activity than penicillin .
	manualset3
168966	3	410444	13	NULL	NULL	0	NULL	ceftriaxone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro activities of penicillin and ceftriaxone were compared against 29 strains of Streptococcus pyogenes with the result that ceftriaxone showed greater activity than penicillin .
	manualset3
168967	4	410444	13	NULL	NULL	0	NULL	29 strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro activities of penicillin and ceftriaxone were compared against 29 strains of Streptococcus pyogenes with the result that ceftriaxone showed greater activity than penicillin .
	manualset3
168968	5	410444	13	NULL	NULL	0	NULL	Streptococcus pyogenes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro activities of penicillin and ceftriaxone were compared against 29 strains of Streptococcus pyogenes with the result that ceftriaxone showed greater activity than penicillin .
	manualset3
168969	6	410444	13	NULL	NULL	0	NULL	result 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro activities of penicillin and ceftriaxone were compared against 29 strains of Streptococcus pyogenes with the result that ceftriaxone showed greater activity than penicillin .
	manualset3
168970	7	410444	13	NULL	NULL	0	NULL	ceftriaxone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro activities of penicillin and ceftriaxone were compared against 29 strains of Streptococcus pyogenes with the result that ceftriaxone showed greater activity than penicillin .
	manualset3
168971	8	410444	13	NULL	NULL	0	NULL	activity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro activities of penicillin and ceftriaxone were compared against 29 strains of Streptococcus pyogenes with the result that ceftriaxone showed greater activity than penicillin .
	manualset3
168972	9	410444	13	NULL	NULL	0	NULL	penicillin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro activities of penicillin and ceftriaxone were compared against 29 strains of Streptococcus pyogenes with the result that ceftriaxone showed greater activity than penicillin .
	manualset3
168973	1	410445	13	NULL	NULL	0	NULL	third member	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A third member of the synapsin gene family .
	manualset3
168974	2	410445	13	NULL	NULL	0	NULL	synapsin gene family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A third member of the synapsin gene family .
	manualset3
168975	1	410446	13	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro binding of warfarin by human serum albumin was studied at various temperatures and at pH 7.4 by a frontal gel filtration technique .
	manualset3
168976	2	410446	13	NULL	NULL	0	NULL	warfarin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro binding of warfarin by human serum albumin was studied at various temperatures and at pH 7.4 by a frontal gel filtration technique .
	manualset3
168977	3	410446	13	NULL	NULL	0	NULL	human serum albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro binding of warfarin by human serum albumin was studied at various temperatures and at pH 7.4 by a frontal gel filtration technique .
	manualset3
168978	4	410446	13	NULL	NULL	0	NULL	temperatures 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro binding of warfarin by human serum albumin was studied at various temperatures and at pH 7.4 by a frontal gel filtration technique .
	manualset3
168979	5	410446	13	NULL	NULL	0	NULL	pH 7.4	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro binding of warfarin by human serum albumin was studied at various temperatures and at pH 7.4 by a frontal gel filtration technique .
	manualset3
168980	6	410446	13	NULL	NULL	0	NULL	frontal gel filtration technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro binding of warfarin by human serum albumin was studied at various temperatures and at pH 7.4 by a frontal gel filtration technique .
	manualset3
168981	1	410447	13	NULL	NULL	0	NULL	dissolution studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro dissolution and in vivo oral absorption studies revealed that the core-shell formulation significantly improved dissolution and absorption behaviors , presumably because of a reduction in particle size , improvement in dispersity , and amorphization .
	manualset3
168982	2	410447	13	NULL	NULL	0	NULL	oral absorption studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro dissolution and in vivo oral absorption studies revealed that the core-shell formulation significantly improved dissolution and absorption behaviors , presumably because of a reduction in particle size , improvement in dispersity , and amorphization .
	manualset3
168983	3	410447	13	NULL	NULL	0	NULL	core-shell formulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro dissolution and in vivo oral absorption studies revealed that the core-shell formulation significantly improved dissolution and absorption behaviors , presumably because of a reduction in particle size , improvement in dispersity , and amorphization .
	manualset3
168984	4	410447	13	NULL	NULL	0	NULL	dissolution behaviors	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro dissolution and in vivo oral absorption studies revealed that the core-shell formulation significantly improved dissolution and absorption behaviors , presumably because of a reduction in particle size , improvement in dispersity , and amorphization .
	manualset3
168985	5	410447	13	NULL	NULL	0	NULL	absorption behaviors	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro dissolution and in vivo oral absorption studies revealed that the core-shell formulation significantly improved dissolution and absorption behaviors , presumably because of a reduction in particle size , improvement in dispersity , and amorphization .
	manualset3
168986	6	410447	13	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro dissolution and in vivo oral absorption studies revealed that the core-shell formulation significantly improved dissolution and absorption behaviors , presumably because of a reduction in particle size , improvement in dispersity , and amorphization .
	manualset3
168987	7	410447	13	NULL	NULL	0	NULL	particle size	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro dissolution and in vivo oral absorption studies revealed that the core-shell formulation significantly improved dissolution and absorption behaviors , presumably because of a reduction in particle size , improvement in dispersity , and amorphization .
	manualset3
168988	8	410447	13	NULL	NULL	0	NULL	improvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro dissolution and in vivo oral absorption studies revealed that the core-shell formulation significantly improved dissolution and absorption behaviors , presumably because of a reduction in particle size , improvement in dispersity , and amorphization .
	manualset3
168989	9	410447	13	NULL	NULL	0	NULL	dispersity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro dissolution and in vivo oral absorption studies revealed that the core-shell formulation significantly improved dissolution and absorption behaviors , presumably because of a reduction in particle size , improvement in dispersity , and amorphization .
	manualset3
168990	10	410447	13	NULL	NULL	0	NULL	amorphization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro dissolution and in vivo oral absorption studies revealed that the core-shell formulation significantly improved dissolution and absorption behaviors , presumably because of a reduction in particle size , improvement in dispersity , and amorphization .
	manualset3
168991	1	410448	13	NULL	NULL	0	NULL	incubations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro incubations of slices of either the transplant or the host 's prostate with testosterone-3H revealed that both tissues could effectively synthesize dihydrotestosterone-3H and androstanediol-3H .
	manualset3
168992	2	410448	13	NULL	NULL	0	NULL	slices 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro incubations of slices of either the transplant or the host 's prostate with testosterone-3H revealed that both tissues could effectively synthesize dihydrotestosterone-3H and androstanediol-3H .
	manualset3
168993	3	410448	13	NULL	NULL	0	NULL	transplant 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro incubations of slices of either the transplant or the host 's prostate with testosterone-3H revealed that both tissues could effectively synthesize dihydrotestosterone-3H and androstanediol-3H .
	manualset3
168994	4	410448	13	NULL	NULL	0	NULL	host 's prostate	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro incubations of slices of either the transplant or the host 's prostate with testosterone-3H revealed that both tissues could effectively synthesize dihydrotestosterone-3H and androstanediol-3H .
	manualset3
168995	5	410448	13	NULL	NULL	0	NULL	testosterone-3H 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro incubations of slices of either the transplant or the host 's prostate with testosterone-3H revealed that both tissues could effectively synthesize dihydrotestosterone-3H and androstanediol-3H .
	manualset3
168996	6	410448	13	NULL	NULL	0	NULL	tissues 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro incubations of slices of either the transplant or the host 's prostate with testosterone-3H revealed that both tissues could effectively synthesize dihydrotestosterone-3H and androstanediol-3H .
	manualset3
168997	7	410448	13	NULL	NULL	0	NULL	dihydrotestosterone-3H	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro incubations of slices of either the transplant or the host 's prostate with testosterone-3H revealed that both tissues could effectively synthesize dihydrotestosterone-3H and androstanediol-3H .
	manualset3
168998	8	410448	13	NULL	NULL	0	NULL	androstanediol-3H 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro incubations of slices of either the transplant or the host 's prostate with testosterone-3H revealed that both tissues could effectively synthesize dihydrotestosterone-3H and androstanediol-3H .
	manualset3
168999	1	410449	13	NULL	NULL	0	NULL	maintenance technique 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro maintenance technique described in this article has been used successfully to rear Cimex lectularius ( L. ) by feeding for ) 2 yr all nymphal stages and adults through parafilm `` M '' sealing film on different types of blood .
	manualset3
169000	2	410449	13	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro maintenance technique described in this article has been used successfully to rear Cimex lectularius ( L. ) by feeding for ) 2 yr all nymphal stages and adults through parafilm `` M '' sealing film on different types of blood .
	manualset3
169001	3	410449	13	NULL	NULL	0	NULL	Cimex lectularius ( L. ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro maintenance technique described in this article has been used successfully to rear Cimex lectularius ( L. ) by feeding for ) 2 yr all nymphal stages and adults through parafilm `` M '' sealing film on different types of blood .
	manualset3
169002	4	410449	13	NULL	NULL	0	NULL	feeding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro maintenance technique described in this article has been used successfully to rear Cimex lectularius ( L. ) by feeding for ) 2 yr all nymphal stages and adults through parafilm `` M '' sealing film on different types of blood .
	manualset3
169003	5	410449	13	NULL	NULL	0	NULL	2 yr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro maintenance technique described in this article has been used successfully to rear Cimex lectularius ( L. ) by feeding for ) 2 yr all nymphal stages and adults through parafilm `` M '' sealing film on different types of blood .
	manualset3
169004	6	410449	13	NULL	NULL	0	NULL	nymphal stages	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro maintenance technique described in this article has been used successfully to rear Cimex lectularius ( L. ) by feeding for ) 2 yr all nymphal stages and adults through parafilm `` M '' sealing film on different types of blood .
	manualset3
169005	7	410449	13	NULL	NULL	0	NULL	adults 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro maintenance technique described in this article has been used successfully to rear Cimex lectularius ( L. ) by feeding for ) 2 yr all nymphal stages and adults through parafilm `` M '' sealing film on different types of blood .
	manualset3
169006	8	410449	13	NULL	NULL	0	NULL	parafilm `` M '' sealing film 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro maintenance technique described in this article has been used successfully to rear Cimex lectularius ( L. ) by feeding for ) 2 yr all nymphal stages and adults through parafilm `` M '' sealing film on different types of blood .
	manualset3
169007	9	410449	13	NULL	NULL	0	NULL	types of blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro maintenance technique described in this article has been used successfully to rear Cimex lectularius ( L. ) by feeding for ) 2 yr all nymphal stages and adults through parafilm `` M '' sealing film on different types of blood .
	manualset3
169008	1	410450	13	NULL	NULL	0	NULL	production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro production of immunoglobulins in response to stimulation with pokeweed mitogen ( PWM ) and fixed/killed Staphylococcus aureus Cowan 1 ( SAC ) was measured in conjunction with in vivo assays of plasma immunoglobulin levels to examine the quality and quantity of humoral immunity during human pregnancy and at parturition .
	manualset3
169009	2	410450	13	NULL	NULL	0	NULL	immunoglobulins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro production of immunoglobulins in response to stimulation with pokeweed mitogen ( PWM ) and fixed/killed Staphylococcus aureus Cowan 1 ( SAC ) was measured in conjunction with in vivo assays of plasma immunoglobulin levels to examine the quality and quantity of humoral immunity during human pregnancy and at parturition .
	manualset3
169010	3	410450	13	NULL	NULL	0	NULL	 response	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro production of immunoglobulins in response to stimulation with pokeweed mitogen ( PWM ) and fixed/killed Staphylococcus aureus Cowan 1 ( SAC ) was measured in conjunction with in vivo assays of plasma immunoglobulin levels to examine the quality and quantity of humoral immunity during human pregnancy and at parturition .
	manualset3
169011	4	410450	13	NULL	NULL	0	NULL	stimulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro production of immunoglobulins in response to stimulation with pokeweed mitogen ( PWM ) and fixed/killed Staphylococcus aureus Cowan 1 ( SAC ) was measured in conjunction with in vivo assays of plasma immunoglobulin levels to examine the quality and quantity of humoral immunity during human pregnancy and at parturition .
	manualset3
169012	5	410450	13	NULL	NULL	0	NULL	pokeweed mitogen ( PWM ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro production of immunoglobulins in response to stimulation with pokeweed mitogen ( PWM ) and fixed/killed Staphylococcus aureus Cowan 1 ( SAC ) was measured in conjunction with in vivo assays of plasma immunoglobulin levels to examine the quality and quantity of humoral immunity during human pregnancy and at parturition .
	manualset3
169013	6	410450	13	NULL	NULL	0	NULL	Staphylococcus aureus Cowan 1 ( SAC )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro production of immunoglobulins in response to stimulation with pokeweed mitogen ( PWM ) and fixed/killed Staphylococcus aureus Cowan 1 ( SAC ) was measured in conjunction with in vivo assays of plasma immunoglobulin levels to examine the quality and quantity of humoral immunity during human pregnancy and at parturition .
	manualset3
169014	7	410450	13	NULL	NULL	0	NULL	conjunction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro production of immunoglobulins in response to stimulation with pokeweed mitogen ( PWM ) and fixed/killed Staphylococcus aureus Cowan 1 ( SAC ) was measured in conjunction with in vivo assays of plasma immunoglobulin levels to examine the quality and quantity of humoral immunity during human pregnancy and at parturition .
	manualset3
169015	8	410450	13	NULL	NULL	0	NULL	in vivo assays 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro production of immunoglobulins in response to stimulation with pokeweed mitogen ( PWM ) and fixed/killed Staphylococcus aureus Cowan 1 ( SAC ) was measured in conjunction with in vivo assays of plasma immunoglobulin levels to examine the quality and quantity of humoral immunity during human pregnancy and at parturition .
	manualset3
169016	9	410450	13	NULL	NULL	0	NULL	plasma immunoglobulin levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro production of immunoglobulins in response to stimulation with pokeweed mitogen ( PWM ) and fixed/killed Staphylococcus aureus Cowan 1 ( SAC ) was measured in conjunction with in vivo assays of plasma immunoglobulin levels to examine the quality and quantity of humoral immunity during human pregnancy and at parturition .
	manualset3
169017	10	410450	13	NULL	NULL	0	NULL	quality 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro production of immunoglobulins in response to stimulation with pokeweed mitogen ( PWM ) and fixed/killed Staphylococcus aureus Cowan 1 ( SAC ) was measured in conjunction with in vivo assays of plasma immunoglobulin levels to examine the quality and quantity of humoral immunity during human pregnancy and at parturition .
	manualset3
169018	11	410450	13	NULL	NULL	0	NULL	quantity 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro production of immunoglobulins in response to stimulation with pokeweed mitogen ( PWM ) and fixed/killed Staphylococcus aureus Cowan 1 ( SAC ) was measured in conjunction with in vivo assays of plasma immunoglobulin levels to examine the quality and quantity of humoral immunity during human pregnancy and at parturition .
	manualset3
169019	12	410450	13	NULL	NULL	0	NULL	humoral immunity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro production of immunoglobulins in response to stimulation with pokeweed mitogen ( PWM ) and fixed/killed Staphylococcus aureus Cowan 1 ( SAC ) was measured in conjunction with in vivo assays of plasma immunoglobulin levels to examine the quality and quantity of humoral immunity during human pregnancy and at parturition .
	manualset3
169020	13	410450	13	NULL	NULL	0	NULL	human pregnancy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro production of immunoglobulins in response to stimulation with pokeweed mitogen ( PWM ) and fixed/killed Staphylococcus aureus Cowan 1 ( SAC ) was measured in conjunction with in vivo assays of plasma immunoglobulin levels to examine the quality and quantity of humoral immunity during human pregnancy and at parturition .
	manualset3
169021	14	410450	13	NULL	NULL	0	NULL	parturition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro production of immunoglobulins in response to stimulation with pokeweed mitogen ( PWM ) and fixed/killed Staphylococcus aureus Cowan 1 ( SAC ) was measured in conjunction with in vivo assays of plasma immunoglobulin levels to examine the quality and quantity of humoral immunity during human pregnancy and at parturition .
	manualset3
169022	1	410451	13	NULL	NULL	0	NULL	release profile	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro release profile of ORI-PLA-NP could be expressed well by the Higuchi equation : Q = 8.944 t ( 1/2 ) +11.246 .
	manualset3
169023	2	410451	13	NULL	NULL	0	NULL	ORI-PLA-NP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro release profile of ORI-PLA-NP could be expressed well by the Higuchi equation : Q = 8.944 t ( 1/2 ) +11.246 .
	manualset3
169024	3	410451	13	NULL	NULL	0	NULL	Higuchi equation	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro release profile of ORI-PLA-NP could be expressed well by the Higuchi equation : Q = 8.944 t ( 1/2 ) +11.246 .
	manualset3
169025	4	410451	13	NULL	NULL	0	NULL	Q = 8.944 t ( 1/2 ) +11.246	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro release profile of ORI-PLA-NP could be expressed well by the Higuchi equation : Q = 8.944 t ( 1/2 ) +11.246 .
	manualset3
169026	1	410452	13	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro results demonstrate that the anticancer activity of camptothecin is significantly enhanced at low drug dose after being encapsulated by these micelles in the presence of serum .
	manualset3
169027	2	410452	13	NULL	NULL	0	NULL	anticancer activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro results demonstrate that the anticancer activity of camptothecin is significantly enhanced at low drug dose after being encapsulated by these micelles in the presence of serum .
	manualset3
169028	3	410452	13	NULL	NULL	0	NULL	camptothecin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro results demonstrate that the anticancer activity of camptothecin is significantly enhanced at low drug dose after being encapsulated by these micelles in the presence of serum .
	manualset3
169029	4	410452	13	NULL	NULL	0	NULL	drug dose	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro results demonstrate that the anticancer activity of camptothecin is significantly enhanced at low drug dose after being encapsulated by these micelles in the presence of serum .
	manualset3
169030	5	410452	13	NULL	NULL	0	NULL	micelles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro results demonstrate that the anticancer activity of camptothecin is significantly enhanced at low drug dose after being encapsulated by these micelles in the presence of serum .
	manualset3
169031	6	410452	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro results demonstrate that the anticancer activity of camptothecin is significantly enhanced at low drug dose after being encapsulated by these micelles in the presence of serum .
	manualset3
169032	7	410452	13	NULL	NULL	0	NULL	serum 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vitro results demonstrate that the anticancer activity of camptothecin is significantly enhanced at low drug dose after being encapsulated by these micelles in the presence of serum .
	manualset3
169033	1	410453	13	NULL	NULL	0	NULL	root box experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vivo root box experiments showed similar Co speciation in the Mn oxide fraction ( 13 to 76 % of total Co ) as the aging and submerged-dried cycling studies .
	manualset3
169034	2	410453	13	NULL	NULL	0	NULL	Co	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vivo root box experiments showed similar Co speciation in the Mn oxide fraction ( 13 to 76 % of total Co ) as the aging and submerged-dried cycling studies .
	manualset3
169035	3	410453	13	NULL	NULL	0	NULL	speciation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vivo root box experiments showed similar Co speciation in the Mn oxide fraction ( 13 to 76 % of total Co ) as the aging and submerged-dried cycling studies .
	manualset3
169036	4	410453	13	NULL	NULL	0	NULL	Mn oxide fraction	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vivo root box experiments showed similar Co speciation in the Mn oxide fraction ( 13 to 76 % of total Co ) as the aging and submerged-dried cycling studies .
	manualset3
169037	5	410453	13	NULL	NULL	0	NULL	13 to 76 % of total Co	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vivo root box experiments showed similar Co speciation in the Mn oxide fraction ( 13 to 76 % of total Co ) as the aging and submerged-dried cycling studies .
	manualset3
169038	6	410453	13	NULL	NULL	0	NULL	submerged-dried cycling studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vivo root box experiments showed similar Co speciation in the Mn oxide fraction ( 13 to 76 % of total Co ) as the aging and submerged-dried cycling studies .
	manualset3
169039	1	410454	13	NULL	NULL	0	NULL	third wave	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A third wave of cell death that was independent of Fig1 and Slt2/Mpk1 was observed in mutants and conditions that eliminate calcineurin signaling .
	manualset3
169040	2	410454	13	NULL	NULL	0	NULL	cell death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A third wave of cell death that was independent of Fig1 and Slt2/Mpk1 was observed in mutants and conditions that eliminate calcineurin signaling .
	manualset3
169041	3	410454	13	NULL	NULL	0	NULL	Fig1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A third wave of cell death that was independent of Fig1 and Slt2/Mpk1 was observed in mutants and conditions that eliminate calcineurin signaling .
	manualset3
169042	4	410454	13	NULL	NULL	0	NULL	Slt2/Mpk1	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A third wave of cell death that was independent of Fig1 and Slt2/Mpk1 was observed in mutants and conditions that eliminate calcineurin signaling .
	manualset3
169043	5	410454	13	NULL	NULL	0	NULL	mutants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A third wave of cell death that was independent of Fig1 and Slt2/Mpk1 was observed in mutants and conditions that eliminate calcineurin signaling .
	manualset3
169044	6	410454	13	NULL	NULL	0	NULL	conditions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A third wave of cell death that was independent of Fig1 and Slt2/Mpk1 was observed in mutants and conditions that eliminate calcineurin signaling .
	manualset3
169045	7	410454	13	NULL	NULL	0	NULL	calcineurin signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A third wave of cell death that was independent of Fig1 and Slt2/Mpk1 was observed in mutants and conditions that eliminate calcineurin signaling .
	manualset3
169091	1	410455	13	NULL	NULL	0	NULL	silico prediction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The in silico prediction was corroborated by studies with the C-3 substituted analog ( methyl at C-3 ) , which showed minimal conversion to CPIC in human liver microsomes .
	manualset3
169092	2	410455	13	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The in silico prediction was corroborated by studies with the C-3 substituted analog ( methyl at C-3 ) , which showed minimal conversion to CPIC in human liver microsomes .
	manualset3
169093	3	410455	13	NULL	NULL	0	NULL	C-3 substituted analog	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The in silico prediction was corroborated by studies with the C-3 substituted analog ( methyl at C-3 ) , which showed minimal conversion to CPIC in human liver microsomes .
	manualset3
169094	4	410455	13	NULL	NULL	0	NULL	methyl at C-3 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The in silico prediction was corroborated by studies with the C-3 substituted analog ( methyl at C-3 ) , which showed minimal conversion to CPIC in human liver microsomes .
	manualset3
169095	5	410455	13	NULL	NULL	0	NULL	conversion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The in silico prediction was corroborated by studies with the C-3 substituted analog ( methyl at C-3 ) , which showed minimal conversion to CPIC in human liver microsomes .
	manualset3
169096	6	410455	13	NULL	NULL	0	NULL	CPIC	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The in silico prediction was corroborated by studies with the C-3 substituted analog ( methyl at C-3 ) , which showed minimal conversion to CPIC in human liver microsomes .
	manualset3
169097	7	410455	13	NULL	NULL	0	NULL	human liver microsomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The in silico prediction was corroborated by studies with the C-3 substituted analog ( methyl at C-3 ) , which showed minimal conversion to CPIC in human liver microsomes .
	manualset3
169098	1	410456	13	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vivo/in vitro studies indicated that the effect of hyperthermia is mainly attributed to radiosensitization , possibly by partial inhibition of sublethal damage repair processes during the subsequent irradiation .
	manualset3
169099	2	410456	13	NULL	NULL	0	NULL	effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vivo/in vitro studies indicated that the effect of hyperthermia is mainly attributed to radiosensitization , possibly by partial inhibition of sublethal damage repair processes during the subsequent irradiation .
	manualset3
169100	3	410456	13	NULL	NULL	0	NULL	hyperthermia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vivo/in vitro studies indicated that the effect of hyperthermia is mainly attributed to radiosensitization , possibly by partial inhibition of sublethal damage repair processes during the subsequent irradiation .
	manualset3
169101	4	410456	13	NULL	NULL	0	NULL	inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vivo/in vitro studies indicated that the effect of hyperthermia is mainly attributed to radiosensitization , possibly by partial inhibition of sublethal damage repair processes during the subsequent irradiation .
	manualset3
169102	5	410456	13	NULL	NULL	0	NULL	sublethal damage repair processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vivo/in vitro studies indicated that the effect of hyperthermia is mainly attributed to radiosensitization , possibly by partial inhibition of sublethal damage repair processes during the subsequent irradiation .
	manualset3
169103	6	410456	13	NULL	NULL	0	NULL	irradiation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vivo/in vitro studies indicated that the effect of hyperthermia is mainly attributed to radiosensitization , possibly by partial inhibition of sublethal damage repair processes during the subsequent irradiation .
	manualset3
178665	7	410456	13	NULL	NULL	0	NULL	radiosensitization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The in vivo/in vitro studies indicated that the effect of hyperthermia is mainly attributed to radiosensitization , possibly by partial inhibition of sublethal damage repair processes during the subsequent irradiation .
	manualset3
169104	1	410457	13	NULL	NULL	0	NULL	inability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The inability to reduce the bacterial burden from the lower respiratory tract within the first few days of therapy for ventilator-associated pneumonia was associated with increased mortality .
	manualset3
169105	2	410457	13	NULL	NULL	0	NULL	bacterial burden	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The inability to reduce the bacterial burden from the lower respiratory tract within the first few days of therapy for ventilator-associated pneumonia was associated with increased mortality .
	manualset3
169106	3	410457	13	NULL	NULL	0	NULL	 lower respiratory tract 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The inability to reduce the bacterial burden from the lower respiratory tract within the first few days of therapy for ventilator-associated pneumonia was associated with increased mortality .
	manualset3
169107	4	410457	13	NULL	NULL	0	NULL	first few days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The inability to reduce the bacterial burden from the lower respiratory tract within the first few days of therapy for ventilator-associated pneumonia was associated with increased mortality .
	manualset3
169108	5	410457	13	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The inability to reduce the bacterial burden from the lower respiratory tract within the first few days of therapy for ventilator-associated pneumonia was associated with increased mortality .
	manualset3
169109	6	410457	13	NULL	NULL	0	NULL	ventilator-associated pneumonia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The inability to reduce the bacterial burden from the lower respiratory tract within the first few days of therapy for ventilator-associated pneumonia was associated with increased mortality .
	manualset3
169110	7	410457	13	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The inability to reduce the bacterial burden from the lower respiratory tract within the first few days of therapy for ventilator-associated pneumonia was associated with increased mortality .
	manualset3
169111	1	410458	13	NULL	NULL	0	NULL	effect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The inactivating effect was shown to be a property of the solid portion of the pus , and was absent from the filtrate .
	manualset3
169112	2	410458	13	NULL	NULL	0	NULL	property	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The inactivating effect was shown to be a property of the solid portion of the pus , and was absent from the filtrate .
	manualset3
169113	3	410458	13	NULL	NULL	0	NULL	solid portion of the pus	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The inactivating effect was shown to be a property of the solid portion of the pus , and was absent from the filtrate .
	manualset3
169114	4	410458	13	NULL	NULL	0	NULL	filtrate	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The inactivating effect was shown to be a property of the solid portion of the pus , and was absent from the filtrate .
	manualset3
169115	1	410459	13	NULL	NULL	0	NULL	incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence and clinical course of this pacemaker complication are unknown .
	manualset3
169116	2	410459	13	NULL	NULL	NULL	NULL	clinical course 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The incidence and clinical course of this pacemaker complication are unknown .
	manualset3
169117	3	410459	13	NULL	NULL	0	NULL	pacemaker complication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence and clinical course of this pacemaker complication are unknown .
	manualset3
169118	1	410460	13	NULL	NULL	0	NULL	incidence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of CMV infection , its severity , timing , and outcome were compared .
	manualset3
169119	2	410460	13	NULL	NULL	0	NULL	CMV infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of CMV infection , its severity , timing , and outcome were compared .
	manualset3
169120	3	410460	13	NULL	NULL	0	NULL	severity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of CMV infection , its severity , timing , and outcome were compared .
	manualset3
169121	4	410460	13	NULL	NULL	0	NULL	timing 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of CMV infection , its severity , timing , and outcome were compared .
	manualset3
169122	5	410460	13	NULL	NULL	0	NULL	outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of CMV infection , its severity , timing , and outcome were compared .
	manualset3
169204	1	410461	13	NULL	NULL	0	NULL	incidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of TIA increased sharply with increasing age , and the overall incidence in men was very similar to that in women ( incidence ratio 1.3 ) .
	manualset3
169205	2	410461	13	NULL	NULL	0	NULL	TIA	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of TIA increased sharply with increasing age , and the overall incidence in men was very similar to that in women ( incidence ratio 1.3 ) .
	manualset3
169206	3	410461	13	NULL	NULL	0	NULL	age 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of TIA increased sharply with increasing age , and the overall incidence in men was very similar to that in women ( incidence ratio 1.3 ) .
	manualset3
169207	4	410461	13	NULL	NULL	0	NULL	incidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of TIA increased sharply with increasing age , and the overall incidence in men was very similar to that in women ( incidence ratio 1.3 ) .
	manualset3
169208	5	410461	13	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of TIA increased sharply with increasing age , and the overall incidence in men was very similar to that in women ( incidence ratio 1.3 ) .
	manualset3
169209	6	410461	13	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of TIA increased sharply with increasing age , and the overall incidence in men was very similar to that in women ( incidence ratio 1.3 ) .
	manualset3
169210	7	410461	13	NULL	NULL	0	NULL	incidence ratio 1.3	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of TIA increased sharply with increasing age , and the overall incidence in men was very similar to that in women ( incidence ratio 1.3 ) .
	manualset3
169211	1	410462	13	NULL	NULL	0	NULL	incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of anxiety and depression was significantly higher in patients than that in controls ( P & lt ; 0.001 ) , and was correlated with the age at which surgery was completed .
	manualset3
169212	2	410462	13	NULL	NULL	0	NULL	anxiety 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of anxiety and depression was significantly higher in patients than that in controls ( P & lt ; 0.001 ) , and was correlated with the age at which surgery was completed .
	manualset3
169213	3	410462	13	NULL	NULL	0	NULL	depression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of anxiety and depression was significantly higher in patients than that in controls ( P & lt ; 0.001 ) , and was correlated with the age at which surgery was completed .
	manualset3
169214	4	410462	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of anxiety and depression was significantly higher in patients than that in controls ( P & lt ; 0.001 ) , and was correlated with the age at which surgery was completed .
	manualset3
169215	5	410462	13	NULL	NULL	0	NULL	controls 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of anxiety and depression was significantly higher in patients than that in controls ( P & lt ; 0.001 ) , and was correlated with the age at which surgery was completed .
	manualset3
169216	6	410462	13	NULL	NULL	0	NULL	P & lt ; 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of anxiety and depression was significantly higher in patients than that in controls ( P & lt ; 0.001 ) , and was correlated with the age at which surgery was completed .
	manualset3
169217	7	410462	13	NULL	NULL	0	NULL	age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of anxiety and depression was significantly higher in patients than that in controls ( P & lt ; 0.001 ) , and was correlated with the age at which surgery was completed .
	manualset3
169218	8	410462	13	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of anxiety and depression was significantly higher in patients than that in controls ( P & lt ; 0.001 ) , and was correlated with the age at which surgery was completed .
	manualset3
169219	1	410463	13	NULL	NULL	0	NULL	thoracoscopic drainage	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A thoracoscopic drainage of pus was performed and antibacterial and antifungal treatment was adapted .
	manualset3
169220	2	410463	13	NULL	NULL	0	NULL	pus	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A thoracoscopic drainage of pus was performed and antibacterial and antifungal treatment was adapted .
	manualset3
169221	3	410463	13	NULL	NULL	0	NULL	antibacterial treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A thoracoscopic drainage of pus was performed and antibacterial and antifungal treatment was adapted .
	manualset3
169222	4	410463	13	NULL	NULL	0	NULL	antifungal treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A thoracoscopic drainage of pus was performed and antibacterial and antifungal treatment was adapted .
	manualset3
169228	1	410464	13	NULL	NULL	0	NULL	incidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of asymptomatic patients had doubled in ten years .
	manualset3
169229	2	410464	13	NULL	NULL	0	NULL	asymptomatic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of asymptomatic patients had doubled in ten years .
	manualset3
169230	3	410464	13	NULL	NULL	0	NULL	ten years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of asymptomatic patients had doubled in ten years .
	manualset3
169231	1	410465	13	NULL	NULL	0	NULL	incidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of capture was not significantly different for pacing algorithms 1-3 .
	manualset3
169232	2	410465	13	NULL	NULL	0	NULL	capture	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of capture was not significantly different for pacing algorithms 1-3 .
	manualset3
169233	3	410465	13	NULL	NULL	0	NULL	algorithms 1-3	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of capture was not significantly different for pacing algorithms 1-3 .
	manualset3
169234	1	410466	13	NULL	NULL	0	NULL	incidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of coronary heart diseases in France is estimated from three sources of information .
	manualset3
169235	2	410466	13	NULL	NULL	0	NULL	coronary heart diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of coronary heart diseases in France is estimated from three sources of information .
	manualset3
169236	3	410466	13	NULL	NULL	0	NULL	France	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of coronary heart diseases in France is estimated from three sources of information .
	manualset3
169237	4	410466	13	NULL	NULL	0	NULL	three sources	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of coronary heart diseases in France is estimated from three sources of information .
	manualset3
169238	5	410466	13	NULL	NULL	0	NULL	information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of coronary heart diseases in France is estimated from three sources of information .
	manualset3
169239	1	410467	13	NULL	NULL	0	NULL	incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of hypercalcemia occurred regardless of the type of phosphate binder containing calcium used , whether it was calcium acetate or calcium carbonate .
	manualset3
169240	2	410467	13	NULL	NULL	0	NULL	hypercalcemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of hypercalcemia occurred regardless of the type of phosphate binder containing calcium used , whether it was calcium acetate or calcium carbonate .
	manualset3
169241	3	410467	13	NULL	NULL	0	NULL	type of phosphate binder	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of hypercalcemia occurred regardless of the type of phosphate binder containing calcium used , whether it was calcium acetate or calcium carbonate .
	manualset3
169242	4	410467	13	NULL	NULL	0	NULL	calcium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of hypercalcemia occurred regardless of the type of phosphate binder containing calcium used , whether it was calcium acetate or calcium carbonate .
	manualset3
169243	5	410467	13	NULL	NULL	0	NULL	calcium acetate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of hypercalcemia occurred regardless of the type of phosphate binder containing calcium used , whether it was calcium acetate or calcium carbonate .
	manualset3
169244	6	410467	13	NULL	NULL	0	NULL	calcium carbonate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of hypercalcemia occurred regardless of the type of phosphate binder containing calcium used , whether it was calcium acetate or calcium carbonate .
	manualset3
169245	1	410468	13	NULL	NULL	0	NULL	incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of ischaemic diseases in familial hypercholesterolemia and xanthomatosis ( familial Type II ) was studied in a group of 158 men and 116 women .
	manualset3
169246	2	410468	13	NULL	NULL	0	NULL	ischaemic diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of ischaemic diseases in familial hypercholesterolemia and xanthomatosis ( familial Type II ) was studied in a group of 158 men and 116 women .
	manualset3
169247	3	410468	13	NULL	NULL	0	NULL	familial hypercholesterolemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of ischaemic diseases in familial hypercholesterolemia and xanthomatosis ( familial Type II ) was studied in a group of 158 men and 116 women .
	manualset3
169248	4	410468	13	NULL	NULL	0	NULL	xanthomatosis ( familial Type II ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of ischaemic diseases in familial hypercholesterolemia and xanthomatosis ( familial Type II ) was studied in a group of 158 men and 116 women .
	manualset3
169249	5	410468	13	NULL	NULL	0	NULL	group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of ischaemic diseases in familial hypercholesterolemia and xanthomatosis ( familial Type II ) was studied in a group of 158 men and 116 women .
	manualset3
169250	6	410468	13	NULL	NULL	0	NULL	158 men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of ischaemic diseases in familial hypercholesterolemia and xanthomatosis ( familial Type II ) was studied in a group of 158 men and 116 women .
	manualset3
169251	7	410468	13	NULL	NULL	0	NULL	116 women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of ischaemic diseases in familial hypercholesterolemia and xanthomatosis ( familial Type II ) was studied in a group of 158 men and 116 women .
	manualset3
169253	1	410469	13	NULL	NULL	0	NULL	incidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of latent fruit infection at the pit hardening stage significantly correlated with that at the late stages and with the incidence of fruit rot at harvest .
	manualset3
169254	2	410469	13	NULL	NULL	0	NULL	latent fruit infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of latent fruit infection at the pit hardening stage significantly correlated with that at the late stages and with the incidence of fruit rot at harvest .
	manualset3
169255	3	410469	13	NULL	NULL	0	NULL	pit hardening stage	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of latent fruit infection at the pit hardening stage significantly correlated with that at the late stages and with the incidence of fruit rot at harvest .
	manualset3
169256	4	410469	13	NULL	NULL	0	NULL	late stages	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of latent fruit infection at the pit hardening stage significantly correlated with that at the late stages and with the incidence of fruit rot at harvest .
	manualset3
169257	5	410469	13	NULL	NULL	0	NULL	incidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of latent fruit infection at the pit hardening stage significantly correlated with that at the late stages and with the incidence of fruit rot at harvest .
	manualset3
169258	6	410469	13	NULL	NULL	0	NULL	fruit rot	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of latent fruit infection at the pit hardening stage significantly correlated with that at the late stages and with the incidence of fruit rot at harvest .
	manualset3
169259	7	410469	13	NULL	NULL	0	NULL	harvest 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of latent fruit infection at the pit hardening stage significantly correlated with that at the late stages and with the incidence of fruit rot at harvest .
	manualset3
169260	1	410470	13	NULL	NULL	0	NULL	incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of mild hyperglycemia ( serum glucose ) 250 mg/dl ) was greater among the rats fed the 25 % protein diet ( 81 % ) than among those fed the 6 % protein diet ( 42 % ) .
	manualset3
169261	2	410470	13	NULL	NULL	0	NULL	mild hyperglycemia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of mild hyperglycemia ( serum glucose ) 250 mg/dl ) was greater among the rats fed the 25 % protein diet ( 81 % ) than among those fed the 6 % protein diet ( 42 % ) .
	manualset3
169262	3	410470	13	NULL	NULL	0	NULL	serum glucose	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of mild hyperglycemia ( serum glucose ) 250 mg/dl ) was greater among the rats fed the 25 % protein diet ( 81 % ) than among those fed the 6 % protein diet ( 42 % ) .
	manualset3
169263	4	410470	13	NULL	NULL	0	NULL	250 mg/dl 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of mild hyperglycemia ( serum glucose ) 250 mg/dl ) was greater among the rats fed the 25 % protein diet ( 81 % ) than among those fed the 6 % protein diet ( 42 % ) .
	manualset3
169264	5	410470	13	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of mild hyperglycemia ( serum glucose ) 250 mg/dl ) was greater among the rats fed the 25 % protein diet ( 81 % ) than among those fed the 6 % protein diet ( 42 % ) .
	manualset3
169265	6	410470	13	NULL	NULL	0	NULL	25 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of mild hyperglycemia ( serum glucose ) 250 mg/dl ) was greater among the rats fed the 25 % protein diet ( 81 % ) than among those fed the 6 % protein diet ( 42 % ) .
	manualset3
169266	7	410470	13	NULL	NULL	0	NULL	protein diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of mild hyperglycemia ( serum glucose ) 250 mg/dl ) was greater among the rats fed the 25 % protein diet ( 81 % ) than among those fed the 6 % protein diet ( 42 % ) .
	manualset3
169267	8	410470	13	NULL	NULL	0	NULL	81 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of mild hyperglycemia ( serum glucose ) 250 mg/dl ) was greater among the rats fed the 25 % protein diet ( 81 % ) than among those fed the 6 % protein diet ( 42 % ) .
	manualset3
169268	9	410470	13	NULL	NULL	NULL	NULL	6 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The incidence of mild hyperglycemia ( serum glucose ) 250 mg/dl ) was greater among the rats fed the 25 % protein diet ( 81 % ) than among those fed the 6 % protein diet ( 42 % ) .
	manualset3
169269	10	410470	13	NULL	NULL	0	NULL	protein diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of mild hyperglycemia ( serum glucose ) 250 mg/dl ) was greater among the rats fed the 25 % protein diet ( 81 % ) than among those fed the 6 % protein diet ( 42 % ) .
	manualset3
169270	11	410470	13	NULL	NULL	0	NULL	42 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of mild hyperglycemia ( serum glucose ) 250 mg/dl ) was greater among the rats fed the 25 % protein diet ( 81 % ) than among those fed the 6 % protein diet ( 42 % ) .
	manualset3
169271	1	410471	13	NULL	NULL	0	NULL	incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of osteoporosis in all subjects increased from 1.13 % in the 21 -- 30-year-old age group to 54.55 % in those over 80 years of age .
	manualset3
169272	2	410471	13	NULL	NULL	0	NULL	osteoporosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of osteoporosis in all subjects increased from 1.13 % in the 21 -- 30-year-old age group to 54.55 % in those over 80 years of age .
	manualset3
169273	3	410471	13	NULL	NULL	0	NULL	subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of osteoporosis in all subjects increased from 1.13 % in the 21 -- 30-year-old age group to 54.55 % in those over 80 years of age .
	manualset3
169274	4	410471	13	NULL	NULL	0	NULL	1.13 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of osteoporosis in all subjects increased from 1.13 % in the 21 -- 30-year-old age group to 54.55 % in those over 80 years of age .
	manualset3
169275	5	410471	13	NULL	NULL	0	NULL	21 -- 30-year-old age group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of osteoporosis in all subjects increased from 1.13 % in the 21 -- 30-year-old age group to 54.55 % in those over 80 years of age .
	manualset3
169276	6	410471	13	NULL	NULL	0	NULL	54.55 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of osteoporosis in all subjects increased from 1.13 % in the 21 -- 30-year-old age group to 54.55 % in those over 80 years of age .
	manualset3
169277	7	410471	13	NULL	NULL	0	NULL	80 years of age 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of osteoporosis in all subjects increased from 1.13 % in the 21 -- 30-year-old age group to 54.55 % in those over 80 years of age .
	manualset3
169278	1	410472	13	NULL	NULL	0	NULL	incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of prostate cancer is age related and increased longevity increases the number of elderly men with the disease .
	manualset3
169279	2	410472	13	NULL	NULL	0	NULL	prostate cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of prostate cancer is age related and increased longevity increases the number of elderly men with the disease .
	manualset3
169280	3	410472	13	NULL	NULL	0	NULL	age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of prostate cancer is age related and increased longevity increases the number of elderly men with the disease .
	manualset3
169281	4	410472	13	NULL	NULL	0	NULL	longevity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of prostate cancer is age related and increased longevity increases the number of elderly men with the disease .
	manualset3
169282	5	410472	13	NULL	NULL	0	NULL	elderly men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of prostate cancer is age related and increased longevity increases the number of elderly men with the disease .
	manualset3
169283	6	410472	13	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of prostate cancer is age related and increased longevity increases the number of elderly men with the disease .
	manualset3
169284	1	410473	13	NULL	NULL	0	NULL	incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of renal angiomyolipoma ( RA ) is 0.3 % in the general population , and even more infrequent during pregnancy .
	manualset3
169285	2	410473	13	NULL	NULL	0	NULL	renal angiomyolipoma ( RA ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of renal angiomyolipoma ( RA ) is 0.3 % in the general population , and even more infrequent during pregnancy .
	manualset3
169286	3	410473	13	NULL	NULL	0	NULL	0.3 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of renal angiomyolipoma ( RA ) is 0.3 % in the general population , and even more infrequent during pregnancy .
	manualset3
169287	4	410473	13	NULL	NULL	0	NULL	general population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of renal angiomyolipoma ( RA ) is 0.3 % in the general population , and even more infrequent during pregnancy .
	manualset3
169288	5	410473	13	NULL	NULL	0	NULL	pregnancy 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of renal angiomyolipoma ( RA ) is 0.3 % in the general population , and even more infrequent during pregnancy .
	manualset3
169289	1	410474	13	NULL	NULL	0	NULL	incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of septic infections was proved to be significantly increased in an extended sample of 100 patients .
	manualset3
169290	2	410474	13	NULL	NULL	0	NULL	septic infections 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of septic infections was proved to be significantly increased in an extended sample of 100 patients .
	manualset3
169291	3	410474	13	NULL	NULL	0	NULL	sample 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of septic infections was proved to be significantly increased in an extended sample of 100 patients .
	manualset3
169292	4	410474	13	NULL	NULL	0	NULL	100 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of septic infections was proved to be significantly increased in an extended sample of 100 patients .
	manualset3
169293	1	410475	13	NULL	NULL	0	NULL	incidence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of transient hypogammaglobulinemia of infancy ( THI ) detected in a major paediatric center over a 10 year period was examined .
	manualset3
169294	2	410475	13	NULL	NULL	0	NULL	transient hypogammaglobulinemia of infancy ( THI ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of transient hypogammaglobulinemia of infancy ( THI ) detected in a major paediatric center over a 10 year period was examined .
	manualset3
169295	3	410475	13	NULL	NULL	NULL	NULL	major paediatric center 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The incidence of transient hypogammaglobulinemia of infancy ( THI ) detected in a major paediatric center over a 10 year period was examined .
	manualset3
169296	4	410475	13	NULL	NULL	0	NULL	10 year period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of transient hypogammaglobulinemia of infancy ( THI ) detected in a major paediatric center over a 10 year period was examined .
	manualset3
169297	1	410476	13	NULL	NULL	0	NULL	incidence rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence rate ( per 1000 person-years ) of dementia , AD and first-ever stroke was 72.3 , 52.2 , and 52.2 in persons with AF and 63.8 , 54.6 and 30.6 in those without AF , respectively .
	manualset3
169298	2	410476	13	NULL	NULL	0	NULL	per 1000 person-years	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence rate ( per 1000 person-years ) of dementia , AD and first-ever stroke was 72.3 , 52.2 , and 52.2 in persons with AF and 63.8 , 54.6 and 30.6 in those without AF , respectively .
	manualset3
169299	3	410476	13	NULL	NULL	0	NULL	dementia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence rate ( per 1000 person-years ) of dementia , AD and first-ever stroke was 72.3 , 52.2 , and 52.2 in persons with AF and 63.8 , 54.6 and 30.6 in those without AF , respectively .
	manualset3
169300	4	410476	13	NULL	NULL	0	NULL	AD 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence rate ( per 1000 person-years ) of dementia , AD and first-ever stroke was 72.3 , 52.2 , and 52.2 in persons with AF and 63.8 , 54.6 and 30.6 in those without AF , respectively .
	manualset3
169301	5	410476	13	NULL	NULL	0	NULL	stroke 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence rate ( per 1000 person-years ) of dementia , AD and first-ever stroke was 72.3 , 52.2 , and 52.2 in persons with AF and 63.8 , 54.6 and 30.6 in those without AF , respectively .
	manualset3
169302	6	410476	13	NULL	NULL	0	NULL	72.3 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence rate ( per 1000 person-years ) of dementia , AD and first-ever stroke was 72.3 , 52.2 , and 52.2 in persons with AF and 63.8 , 54.6 and 30.6 in those without AF , respectively .
	manualset3
169303	7	410476	13	NULL	NULL	0	NULL	52.2 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence rate ( per 1000 person-years ) of dementia , AD and first-ever stroke was 72.3 , 52.2 , and 52.2 in persons with AF and 63.8 , 54.6 and 30.6 in those without AF , respectively .
	manualset3
169304	8	410476	13	NULL	NULL	0	NULL	52.2 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence rate ( per 1000 person-years ) of dementia , AD and first-ever stroke was 72.3 , 52.2 , and 52.2 in persons with AF and 63.8 , 54.6 and 30.6 in those without AF , respectively .
	manualset3
169305	9	410476	13	NULL	NULL	0	NULL	persons 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence rate ( per 1000 person-years ) of dementia , AD and first-ever stroke was 72.3 , 52.2 , and 52.2 in persons with AF and 63.8 , 54.6 and 30.6 in those without AF , respectively .
	manualset3
169306	10	410476	13	NULL	NULL	0	NULL	AF 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence rate ( per 1000 person-years ) of dementia , AD and first-ever stroke was 72.3 , 52.2 , and 52.2 in persons with AF and 63.8 , 54.6 and 30.6 in those without AF , respectively .
	manualset3
169307	11	410476	13	NULL	NULL	0	NULL	63.8 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence rate ( per 1000 person-years ) of dementia , AD and first-ever stroke was 72.3 , 52.2 , and 52.2 in persons with AF and 63.8 , 54.6 and 30.6 in those without AF , respectively .
	manualset3
169308	12	410476	13	NULL	NULL	0	NULL	54.6 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence rate ( per 1000 person-years ) of dementia , AD and first-ever stroke was 72.3 , 52.2 , and 52.2 in persons with AF and 63.8 , 54.6 and 30.6 in those without AF , respectively .
	manualset3
169309	13	410476	13	NULL	NULL	0	NULL	30.6 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence rate ( per 1000 person-years ) of dementia , AD and first-ever stroke was 72.3 , 52.2 , and 52.2 in persons with AF and 63.8 , 54.6 and 30.6 in those without AF , respectively .
	manualset3
169310	14	410476	13	NULL	NULL	0	NULL	AF 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence rate ( per 1000 person-years ) of dementia , AD and first-ever stroke was 72.3 , 52.2 , and 52.2 in persons with AF and 63.8 , 54.6 and 30.6 in those without AF , respectively .
	manualset3
169311	1	410477	13	NULL	NULL	0	NULL	incidence rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence rate of system and target organ disorders as a total of all production plants was 6 % on average over the 3-year period , and for laboratory workers it was 10.3 % .
	manualset3
169312	2	410477	13	NULL	NULL	0	NULL	system 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence rate of system and target organ disorders as a total of all production plants was 6 % on average over the 3-year period , and for laboratory workers it was 10.3 % .
	manualset3
169313	3	410477	13	NULL	NULL	0	NULL	target organ disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence rate of system and target organ disorders as a total of all production plants was 6 % on average over the 3-year period , and for laboratory workers it was 10.3 % .
	manualset3
169314	4	410477	13	NULL	NULL	0	NULL	total 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence rate of system and target organ disorders as a total of all production plants was 6 % on average over the 3-year period , and for laboratory workers it was 10.3 % .
	manualset3
169315	5	410477	13	NULL	NULL	0	NULL	production plants 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence rate of system and target organ disorders as a total of all production plants was 6 % on average over the 3-year period , and for laboratory workers it was 10.3 % .
	manualset3
169316	6	410477	13	NULL	NULL	0	NULL	6 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence rate of system and target organ disorders as a total of all production plants was 6 % on average over the 3-year period , and for laboratory workers it was 10.3 % .
	manualset3
169317	7	410477	13	NULL	NULL	0	NULL	average 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence rate of system and target organ disorders as a total of all production plants was 6 % on average over the 3-year period , and for laboratory workers it was 10.3 % .
	manualset3
169318	8	410477	13	NULL	NULL	0	NULL	3-year period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence rate of system and target organ disorders as a total of all production plants was 6 % on average over the 3-year period , and for laboratory workers it was 10.3 % .
	manualset3
169319	9	410477	13	NULL	NULL	0	NULL	laboratory workers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence rate of system and target organ disorders as a total of all production plants was 6 % on average over the 3-year period , and for laboratory workers it was 10.3 % .
	manualset3
169320	10	410477	13	NULL	NULL	0	NULL	10.3 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence rate of system and target organ disorders as a total of all production plants was 6 % on average over the 3-year period , and for laboratory workers it was 10.3 % .
	manualset3
169323	1	410478	13	NULL	NULL	0	NULL	inclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The inclusion criteria used were : randomized trial , radiolucent gallstones in a visualizing gallbladder on oral cholecystography , and complete stone dissolution confirmed by oral cholecystography or ultrasound .
	manualset3
169324	2	410478	13	NULL	NULL	0	NULL	criteria	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The inclusion criteria used were : randomized trial , radiolucent gallstones in a visualizing gallbladder on oral cholecystography , and complete stone dissolution confirmed by oral cholecystography or ultrasound .
	manualset3
169325	3	410478	13	NULL	NULL	NULL	NULL	randomized trial	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The inclusion criteria used were : randomized trial , radiolucent gallstones in a visualizing gallbladder on oral cholecystography , and complete stone dissolution confirmed by oral cholecystography or ultrasound .
	manualset3
169326	4	410478	13	NULL	NULL	0	NULL	radiolucent gallstones	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The inclusion criteria used were : randomized trial , radiolucent gallstones in a visualizing gallbladder on oral cholecystography , and complete stone dissolution confirmed by oral cholecystography or ultrasound .
	manualset3
169327	5	410478	13	NULL	NULL	0	NULL	gallbladder	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The inclusion criteria used were : randomized trial , radiolucent gallstones in a visualizing gallbladder on oral cholecystography , and complete stone dissolution confirmed by oral cholecystography or ultrasound .
	manualset3
169328	6	410478	13	NULL	NULL	0	NULL	oral cholecystography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The inclusion criteria used were : randomized trial , radiolucent gallstones in a visualizing gallbladder on oral cholecystography , and complete stone dissolution confirmed by oral cholecystography or ultrasound .
	manualset3
169329	7	410478	13	NULL	NULL	0	NULL	complete stone dissolution	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The inclusion criteria used were : randomized trial , radiolucent gallstones in a visualizing gallbladder on oral cholecystography , and complete stone dissolution confirmed by oral cholecystography or ultrasound .
	manualset3
169330	8	410478	13	NULL	NULL	0	NULL	oral cholecystography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The inclusion criteria used were : randomized trial , radiolucent gallstones in a visualizing gallbladder on oral cholecystography , and complete stone dissolution confirmed by oral cholecystography or ultrasound .
	manualset3
169331	9	410478	13	NULL	NULL	0	NULL	ultrasound	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The inclusion criteria used were : randomized trial , radiolucent gallstones in a visualizing gallbladder on oral cholecystography , and complete stone dissolution confirmed by oral cholecystography or ultrasound .
	manualset3
169332	1	410479	13	NULL	NULL	0	NULL	inclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The inclusion of beta-cyclodextrin ( CD ) for thionine ( TH ) and the interaction of DNA with CD-TH inclusion complex were investigated by fluorescence and visible absorption spectrometry .
	manualset3
169333	2	410479	13	NULL	NULL	0	NULL	beta-cyclodextrin ( CD )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The inclusion of beta-cyclodextrin ( CD ) for thionine ( TH ) and the interaction of DNA with CD-TH inclusion complex were investigated by fluorescence and visible absorption spectrometry .
	manualset3
169334	3	410479	13	NULL	NULL	0	NULL	thionine ( TH )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The inclusion of beta-cyclodextrin ( CD ) for thionine ( TH ) and the interaction of DNA with CD-TH inclusion complex were investigated by fluorescence and visible absorption spectrometry .
	manualset3
169335	4	410479	13	NULL	NULL	0	NULL	interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The inclusion of beta-cyclodextrin ( CD ) for thionine ( TH ) and the interaction of DNA with CD-TH inclusion complex were investigated by fluorescence and visible absorption spectrometry .
	manualset3
169336	5	410479	13	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The inclusion of beta-cyclodextrin ( CD ) for thionine ( TH ) and the interaction of DNA with CD-TH inclusion complex were investigated by fluorescence and visible absorption spectrometry .
	manualset3
169337	6	410479	13	NULL	NULL	0	NULL	CD-TH inclusion complex	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The inclusion of beta-cyclodextrin ( CD ) for thionine ( TH ) and the interaction of DNA with CD-TH inclusion complex were investigated by fluorescence and visible absorption spectrometry .
	manualset3
169338	7	410479	13	NULL	NULL	0	NULL	fluorescence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The inclusion of beta-cyclodextrin ( CD ) for thionine ( TH ) and the interaction of DNA with CD-TH inclusion complex were investigated by fluorescence and visible absorption spectrometry .
	manualset3
169339	8	410479	13	NULL	NULL	0	NULL	visible absorption spectrometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The inclusion of beta-cyclodextrin ( CD ) for thionine ( TH ) and the interaction of DNA with CD-TH inclusion complex were investigated by fluorescence and visible absorption spectrometry .
	manualset3
169344	1	410480	13	NULL	NULL	0	NULL	inclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The inclusion of boxes 6 , 7 was associated with a significant decrease in the binding of FAK + to the c-Src and Fyn SH3 domains , and a significant increase in the binding to the Src SH2 domain , as a consequence of the higher phosphorylation of Tyr-397 .
	manualset3
169345	2	410480	13	NULL	NULL	0	NULL	boxes 6 , 7	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The inclusion of boxes 6 , 7 was associated with a significant decrease in the binding of FAK + to the c-Src and Fyn SH3 domains , and a significant increase in the binding to the Src SH2 domain , as a consequence of the higher phosphorylation of Tyr-397 .
	manualset3
169346	3	410480	13	NULL	NULL	0	NULL	decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The inclusion of boxes 6 , 7 was associated with a significant decrease in the binding of FAK + to the c-Src and Fyn SH3 domains , and a significant increase in the binding to the Src SH2 domain , as a consequence of the higher phosphorylation of Tyr-397 .
	manualset3
169347	4	410480	13	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The inclusion of boxes 6 , 7 was associated with a significant decrease in the binding of FAK + to the c-Src and Fyn SH3 domains , and a significant increase in the binding to the Src SH2 domain , as a consequence of the higher phosphorylation of Tyr-397 .
	manualset3
169348	5	410480	13	NULL	NULL	0	NULL	FAK +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The inclusion of boxes 6 , 7 was associated with a significant decrease in the binding of FAK + to the c-Src and Fyn SH3 domains , and a significant increase in the binding to the Src SH2 domain , as a consequence of the higher phosphorylation of Tyr-397 .
	manualset3
169349	6	410480	13	NULL	NULL	0	NULL	c-Src SH3 domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The inclusion of boxes 6 , 7 was associated with a significant decrease in the binding of FAK + to the c-Src and Fyn SH3 domains , and a significant increase in the binding to the Src SH2 domain , as a consequence of the higher phosphorylation of Tyr-397 .
	manualset3
169350	7	410480	13	NULL	NULL	0	NULL	Fyn SH3 domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The inclusion of boxes 6 , 7 was associated with a significant decrease in the binding of FAK + to the c-Src and Fyn SH3 domains , and a significant increase in the binding to the Src SH2 domain , as a consequence of the higher phosphorylation of Tyr-397 .
	manualset3
169351	8	410480	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The inclusion of boxes 6 , 7 was associated with a significant decrease in the binding of FAK + to the c-Src and Fyn SH3 domains , and a significant increase in the binding to the Src SH2 domain , as a consequence of the higher phosphorylation of Tyr-397 .
	manualset3
169352	9	410480	13	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The inclusion of boxes 6 , 7 was associated with a significant decrease in the binding of FAK + to the c-Src and Fyn SH3 domains , and a significant increase in the binding to the Src SH2 domain , as a consequence of the higher phosphorylation of Tyr-397 .
	manualset3
169353	10	410480	13	NULL	NULL	0	NULL	Src SH2 domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The inclusion of boxes 6 , 7 was associated with a significant decrease in the binding of FAK + to the c-Src and Fyn SH3 domains , and a significant increase in the binding to the Src SH2 domain , as a consequence of the higher phosphorylation of Tyr-397 .
	manualset3
169354	11	410480	13	NULL	NULL	0	NULL	consequence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The inclusion of boxes 6 , 7 was associated with a significant decrease in the binding of FAK + to the c-Src and Fyn SH3 domains , and a significant increase in the binding to the Src SH2 domain , as a consequence of the higher phosphorylation of Tyr-397 .
	manualset3
169355	12	410480	13	NULL	NULL	0	NULL	phosphorylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The inclusion of boxes 6 , 7 was associated with a significant decrease in the binding of FAK + to the c-Src and Fyn SH3 domains , and a significant increase in the binding to the Src SH2 domain , as a consequence of the higher phosphorylation of Tyr-397 .
	manualset3
169356	13	410480	13	NULL	NULL	0	NULL	Tyr-397	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The inclusion of boxes 6 , 7 was associated with a significant decrease in the binding of FAK + to the c-Src and Fyn SH3 domains , and a significant increase in the binding to the Src SH2 domain , as a consequence of the higher phosphorylation of Tyr-397 .
	manualset3
169357	1	410481	13	NULL	NULL	0	NULL	transcripts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The incomplete transcripts were represented by many distinct bands , pointing to the presence of multiple stops in the process of elongation .
	manualset3
169358	2	410481	13	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The incomplete transcripts were represented by many distinct bands , pointing to the presence of multiple stops in the process of elongation .
	manualset3
169359	3	410481	13	NULL	NULL	0	NULL	multiple stops	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The incomplete transcripts were represented by many distinct bands , pointing to the presence of multiple stops in the process of elongation .
	manualset3
169360	4	410481	13	NULL	NULL	0	NULL	process	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The incomplete transcripts were represented by many distinct bands , pointing to the presence of multiple stops in the process of elongation .
	manualset3
169361	5	410481	13	NULL	NULL	0	NULL	elongation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The incomplete transcripts were represented by many distinct bands , pointing to the presence of multiple stops in the process of elongation .
	manualset3
169362	6	410481	13	NULL	NULL	0	NULL	distinct bands	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The incomplete transcripts were represented by many distinct bands , pointing to the presence of multiple stops in the process of elongation .
	manualset3
169363	1	410482	13	NULL	NULL	0	NULL	incontinence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The incontinence was severer in the patients with the tumors of pT3 or pT4 than in the patients with the tumors of pT2 .
	manualset3
169364	2	410482	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The incontinence was severer in the patients with the tumors of pT3 or pT4 than in the patients with the tumors of pT2 .
	manualset3
169365	3	410482	13	NULL	NULL	0	NULL	tumors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incontinence was severer in the patients with the tumors of pT3 or pT4 than in the patients with the tumors of pT2 .
	manualset3
169366	4	410482	13	NULL	NULL	0	NULL	pT3 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incontinence was severer in the patients with the tumors of pT3 or pT4 than in the patients with the tumors of pT2 .
	manualset3
169367	5	410482	13	NULL	NULL	0	NULL	pT4 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incontinence was severer in the patients with the tumors of pT3 or pT4 than in the patients with the tumors of pT2 .
	manualset3
169368	6	410482	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The incontinence was severer in the patients with the tumors of pT3 or pT4 than in the patients with the tumors of pT2 .
	manualset3
169369	7	410482	13	NULL	NULL	0	NULL	tumors of pT2	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incontinence was severer in the patients with the tumors of pT3 or pT4 than in the patients with the tumors of pT2 .
	manualset3
169370	1	410483	13	NULL	NULL	0	NULL	incorporation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The incorporation of JPEG 2000 within the DICOM standard does little to guarantee its longevity , or the quality of every JPEG 2000 implementation .
	manualset3
169371	2	410483	13	NULL	NULL	0	NULL	JPEG 2000	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The incorporation of JPEG 2000 within the DICOM standard does little to guarantee its longevity , or the quality of every JPEG 2000 implementation .
	manualset3
169372	3	410483	13	NULL	NULL	0	NULL	DICOM standard 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The incorporation of JPEG 2000 within the DICOM standard does little to guarantee its longevity , or the quality of every JPEG 2000 implementation .
	manualset3
169373	4	410483	13	NULL	NULL	0	NULL	longevity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The incorporation of JPEG 2000 within the DICOM standard does little to guarantee its longevity , or the quality of every JPEG 2000 implementation .
	manualset3
169374	5	410483	13	NULL	NULL	0	NULL	quality 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The incorporation of JPEG 2000 within the DICOM standard does little to guarantee its longevity , or the quality of every JPEG 2000 implementation .
	manualset3
169375	6	410483	13	NULL	NULL	0	NULL	JPEG 2000 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The incorporation of JPEG 2000 within the DICOM standard does little to guarantee its longevity , or the quality of every JPEG 2000 implementation .
	manualset3
169376	7	410483	13	NULL	NULL	0	NULL	implementation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The incorporation of JPEG 2000 within the DICOM standard does little to guarantee its longevity , or the quality of every JPEG 2000 implementation .
	manualset3
169377	1	410484	13	NULL	NULL	0	NULL	features 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The incorporation/exclusion features of dopamine ( DA ) , ascorbic acid ( AA ) and uric acid ( UA ) are evaluated for Nafion ( NA ) - coated glassy carbon electrodes ( GCE ) of different thicknesses .
	manualset3
169378	2	410484	13	NULL	NULL	0	NULL	dopamine ( DA ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The incorporation/exclusion features of dopamine ( DA ) , ascorbic acid ( AA ) and uric acid ( UA ) are evaluated for Nafion ( NA ) - coated glassy carbon electrodes ( GCE ) of different thicknesses .
	manualset3
169379	3	410484	13	NULL	NULL	0	NULL	ascorbic acid ( AA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The incorporation/exclusion features of dopamine ( DA ) , ascorbic acid ( AA ) and uric acid ( UA ) are evaluated for Nafion ( NA ) - coated glassy carbon electrodes ( GCE ) of different thicknesses .
	manualset3
169380	4	410484	13	NULL	NULL	0	NULL	uric acid ( UA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The incorporation/exclusion features of dopamine ( DA ) , ascorbic acid ( AA ) and uric acid ( UA ) are evaluated for Nafion ( NA ) - coated glassy carbon electrodes ( GCE ) of different thicknesses .
	manualset3
169381	5	410484	13	NULL	NULL	0	NULL	Nafion ( NA ) - coated glassy carbon electrodes ( GCE )	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The incorporation/exclusion features of dopamine ( DA ) , ascorbic acid ( AA ) and uric acid ( UA ) are evaluated for Nafion ( NA ) - coated glassy carbon electrodes ( GCE ) of different thicknesses .
	manualset3
169382	6	410484	13	NULL	NULL	0	NULL	thicknesses	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The incorporation/exclusion features of dopamine ( DA ) , ascorbic acid ( AA ) and uric acid ( UA ) are evaluated for Nafion ( NA ) - coated glassy carbon electrodes ( GCE ) of different thicknesses .
	manualset3
169383	1	410485	13	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in AaDo2 after placebo was significant , but that after tiapamil was not .
	manualset3
169384	2	410485	13	NULL	NULL	0	NULL	AaDo2 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in AaDo2 after placebo was significant , but that after tiapamil was not .
	manualset3
169385	3	410485	13	NULL	NULL	0	NULL	placebo 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in AaDo2 after placebo was significant , but that after tiapamil was not .
	manualset3
169386	4	410485	13	NULL	NULL	0	NULL	tiapamil 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in AaDo2 after placebo was significant , but that after tiapamil was not .
	manualset3
169387	1	410486	13	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in Zn content occurred simultaneously with the increase in Cd concentration in the liver ( Zn to Cd ratio was 1 : 1 ) .
	manualset3
169388	2	410486	13	NULL	NULL	0	NULL	Zn 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in Zn content occurred simultaneously with the increase in Cd concentration in the liver ( Zn to Cd ratio was 1 : 1 ) .
	manualset3
169389	3	410486	13	NULL	NULL	0	NULL	content 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in Zn content occurred simultaneously with the increase in Cd concentration in the liver ( Zn to Cd ratio was 1 : 1 ) .
	manualset3
169390	4	410486	13	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in Zn content occurred simultaneously with the increase in Cd concentration in the liver ( Zn to Cd ratio was 1 : 1 ) .
	manualset3
169391	5	410486	13	NULL	NULL	0	NULL	Cd 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in Zn content occurred simultaneously with the increase in Cd concentration in the liver ( Zn to Cd ratio was 1 : 1 ) .
	manualset3
169392	6	410486	13	NULL	NULL	0	NULL	concentration 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in Zn content occurred simultaneously with the increase in Cd concentration in the liver ( Zn to Cd ratio was 1 : 1 ) .
	manualset3
169393	7	410486	13	NULL	NULL	0	NULL	liver 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in Zn content occurred simultaneously with the increase in Cd concentration in the liver ( Zn to Cd ratio was 1 : 1 ) .
	manualset3
169394	8	410486	13	NULL	NULL	0	NULL	Zn 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in Zn content occurred simultaneously with the increase in Cd concentration in the liver ( Zn to Cd ratio was 1 : 1 ) .
	manualset3
169395	9	410486	13	NULL	NULL	0	NULL	Cd 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in Zn content occurred simultaneously with the increase in Cd concentration in the liver ( Zn to Cd ratio was 1 : 1 ) .
	manualset3
169396	10	410486	13	NULL	NULL	0	NULL	ratio 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in Zn content occurred simultaneously with the increase in Cd concentration in the liver ( Zn to Cd ratio was 1 : 1 ) .
	manualset3
169397	11	410486	13	NULL	NULL	0	NULL	1 : 1 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in Zn content occurred simultaneously with the increase in Cd concentration in the liver ( Zn to Cd ratio was 1 : 1 ) .
	manualset3
169398	1	410487	13	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in bodyweight observed in November was due to accumulation of white adipose tissue in the posterior abdominal region .
	manualset3
169399	2	410487	13	NULL	NULL	0	NULL	bodyweight 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in bodyweight observed in November was due to accumulation of white adipose tissue in the posterior abdominal region .
	manualset3
169400	3	410487	13	NULL	NULL	0	NULL	November 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in bodyweight observed in November was due to accumulation of white adipose tissue in the posterior abdominal region .
	manualset3
169401	4	410487	13	NULL	NULL	0	NULL	accumulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in bodyweight observed in November was due to accumulation of white adipose tissue in the posterior abdominal region .
	manualset3
169402	5	410487	13	NULL	NULL	0	NULL	white adipose tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in bodyweight observed in November was due to accumulation of white adipose tissue in the posterior abdominal region .
	manualset3
169403	6	410487	13	NULL	NULL	0	NULL	posterior abdominal region 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in bodyweight observed in November was due to accumulation of white adipose tissue in the posterior abdominal region .
	manualset3
169404	1	410488	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in cholesterol in women with the APOE3E4 genotype did not differ from the increase in women with the APOE3E3 genotype .
	manualset3
169405	2	410488	13	NULL	NULL	0	NULL	cholesterol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in cholesterol in women with the APOE3E4 genotype did not differ from the increase in women with the APOE3E3 genotype .
	manualset3
169406	3	410488	13	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in cholesterol in women with the APOE3E4 genotype did not differ from the increase in women with the APOE3E3 genotype .
	manualset3
169407	4	410488	13	NULL	NULL	0	NULL	APOE3E4 genotype	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in cholesterol in women with the APOE3E4 genotype did not differ from the increase in women with the APOE3E3 genotype .
	manualset3
169408	5	410488	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in cholesterol in women with the APOE3E4 genotype did not differ from the increase in women with the APOE3E3 genotype .
	manualset3
169409	6	410488	13	NULL	NULL	0	NULL	women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in cholesterol in women with the APOE3E4 genotype did not differ from the increase in women with the APOE3E3 genotype .
	manualset3
169410	7	410488	13	NULL	NULL	0	NULL	APOE3E3 genotype	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in cholesterol in women with the APOE3E4 genotype did not differ from the increase in women with the APOE3E3 genotype .
	manualset3
169411	1	410489	13	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in strength correlated ( P less than 0.05 ) with significant ( P less than 0.05-0 .01 ) increases in the neural activation ( IEMG ) of the leg extensor muscles during the most intensive training months .
	manualset3
169412	2	410489	13	NULL	NULL	0	NULL	strength 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in strength correlated ( P less than 0.05 ) with significant ( P less than 0.05-0 .01 ) increases in the neural activation ( IEMG ) of the leg extensor muscles during the most intensive training months .
	manualset3
169413	3	410489	13	NULL	NULL	0	NULL	P less than 0.05 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in strength correlated ( P less than 0.05 ) with significant ( P less than 0.05-0 .01 ) increases in the neural activation ( IEMG ) of the leg extensor muscles during the most intensive training months .
	manualset3
169414	4	410489	13	NULL	NULL	0	NULL	P less than 0.05-0 .01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in strength correlated ( P less than 0.05 ) with significant ( P less than 0.05-0 .01 ) increases in the neural activation ( IEMG ) of the leg extensor muscles during the most intensive training months .
	manualset3
169415	5	410489	13	NULL	NULL	0	NULL	increases 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in strength correlated ( P less than 0.05 ) with significant ( P less than 0.05-0 .01 ) increases in the neural activation ( IEMG ) of the leg extensor muscles during the most intensive training months .
	manualset3
169416	6	410489	13	NULL	NULL	0	NULL	neural activation ( IEMG )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in strength correlated ( P less than 0.05 ) with significant ( P less than 0.05-0 .01 ) increases in the neural activation ( IEMG ) of the leg extensor muscles during the most intensive training months .
	manualset3
169417	7	410489	13	NULL	NULL	0	NULL	leg extensor muscles 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in strength correlated ( P less than 0.05 ) with significant ( P less than 0.05-0 .01 ) increases in the neural activation ( IEMG ) of the leg extensor muscles during the most intensive training months .
	manualset3
169418	8	410489	13	NULL	NULL	0	NULL	training months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in strength correlated ( P less than 0.05 ) with significant ( P less than 0.05-0 .01 ) increases in the neural activation ( IEMG ) of the leg extensor muscles during the most intensive training months .
	manualset3
169419	1	410490	13	NULL	NULL	0	NULL	total	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 1 968 persons aged 18-20 years belonging to organized groups were immunized with different doses of polysaccharide meningococcal divaccine , groups A and C , by means of syringes and jet injectors under the conditions of a controlled epidemiological trial .
	manualset3
169420	2	410490	13	NULL	NULL	0	NULL	1 968 persons	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 1 968 persons aged 18-20 years belonging to organized groups were immunized with different doses of polysaccharide meningococcal divaccine , groups A and C , by means of syringes and jet injectors under the conditions of a controlled epidemiological trial .
	manualset3
169421	3	410490	13	NULL	NULL	0	NULL	aged 18-20 years	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 1 968 persons aged 18-20 years belonging to organized groups were immunized with different doses of polysaccharide meningococcal divaccine , groups A and C , by means of syringes and jet injectors under the conditions of a controlled epidemiological trial .
	manualset3
169422	4	410490	13	NULL	NULL	0	NULL	organized groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 1 968 persons aged 18-20 years belonging to organized groups were immunized with different doses of polysaccharide meningococcal divaccine , groups A and C , by means of syringes and jet injectors under the conditions of a controlled epidemiological trial .
	manualset3
169423	5	410490	13	NULL	NULL	0	NULL	doses	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 1 968 persons aged 18-20 years belonging to organized groups were immunized with different doses of polysaccharide meningococcal divaccine , groups A and C , by means of syringes and jet injectors under the conditions of a controlled epidemiological trial .
	manualset3
169424	6	410490	13	NULL	NULL	0	NULL	polysaccharide meningococcal divaccine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 1 968 persons aged 18-20 years belonging to organized groups were immunized with different doses of polysaccharide meningococcal divaccine , groups A and C , by means of syringes and jet injectors under the conditions of a controlled epidemiological trial .
	manualset3
169425	7	410490	13	NULL	NULL	0	NULL	groups A	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 1 968 persons aged 18-20 years belonging to organized groups were immunized with different doses of polysaccharide meningococcal divaccine , groups A and C , by means of syringes and jet injectors under the conditions of a controlled epidemiological trial .
	manualset3
169426	8	410490	13	NULL	NULL	0	NULL	groups C	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 1 968 persons aged 18-20 years belonging to organized groups were immunized with different doses of polysaccharide meningococcal divaccine , groups A and C , by means of syringes and jet injectors under the conditions of a controlled epidemiological trial .
	manualset3
169427	9	410490	13	NULL	NULL	0	NULL	syringes	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 1 968 persons aged 18-20 years belonging to organized groups were immunized with different doses of polysaccharide meningococcal divaccine , groups A and C , by means of syringes and jet injectors under the conditions of a controlled epidemiological trial .
	manualset3
169428	10	410490	13	NULL	NULL	0	NULL	jet injectors 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 1 968 persons aged 18-20 years belonging to organized groups were immunized with different doses of polysaccharide meningococcal divaccine , groups A and C , by means of syringes and jet injectors under the conditions of a controlled epidemiological trial .
	manualset3
169429	11	410490	13	NULL	NULL	0	NULL	conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 1 968 persons aged 18-20 years belonging to organized groups were immunized with different doses of polysaccharide meningococcal divaccine , groups A and C , by means of syringes and jet injectors under the conditions of a controlled epidemiological trial .
	manualset3
169430	12	410490	13	NULL	NULL	0	NULL	epidemiological trial 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 1 968 persons aged 18-20 years belonging to organized groups were immunized with different doses of polysaccharide meningococcal divaccine , groups A and C , by means of syringes and jet injectors under the conditions of a controlled epidemiological trial .
	manualset3
169431	13	410490	13	NULL	NULL	0	NULL	means	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 1 968 persons aged 18-20 years belonging to organized groups were immunized with different doses of polysaccharide meningococcal divaccine , groups A and C , by means of syringes and jet injectors under the conditions of a controlled epidemiological trial .
	manualset3
169432	1	410491	13	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in survival time produced by the immunotherapy is apparently made up of two components : prolongation of the first remission and length of survival after the first relapse .
	manualset3
169433	2	410491	13	NULL	NULL	0	NULL	survival time	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in survival time produced by the immunotherapy is apparently made up of two components : prolongation of the first remission and length of survival after the first relapse .
	manualset3
169434	3	410491	13	NULL	NULL	0	NULL	immunotherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in survival time produced by the immunotherapy is apparently made up of two components : prolongation of the first remission and length of survival after the first relapse .
	manualset3
169435	4	410491	13	NULL	NULL	0	NULL	two components	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in survival time produced by the immunotherapy is apparently made up of two components : prolongation of the first remission and length of survival after the first relapse .
	manualset3
169436	5	410491	13	NULL	NULL	0	NULL	prolongation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in survival time produced by the immunotherapy is apparently made up of two components : prolongation of the first remission and length of survival after the first relapse .
	manualset3
169437	6	410491	13	NULL	NULL	0	NULL	first remission	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in survival time produced by the immunotherapy is apparently made up of two components : prolongation of the first remission and length of survival after the first relapse .
	manualset3
169438	7	410491	13	NULL	NULL	0	NULL	length of survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in survival time produced by the immunotherapy is apparently made up of two components : prolongation of the first remission and length of survival after the first relapse .
	manualset3
169439	8	410491	13	NULL	NULL	0	NULL	first relapse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in survival time produced by the immunotherapy is apparently made up of two components : prolongation of the first remission and length of survival after the first relapse .
	manualset3
169440	1	410492	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in the relative risk of pancreatic cancer was similar in former and current snus users and was restricted to current tobacco smokers .
	manualset3
169441	2	410492	13	NULL	NULL	0	NULL	relative risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in the relative risk of pancreatic cancer was similar in former and current snus users and was restricted to current tobacco smokers .
	manualset3
169442	3	410492	13	NULL	NULL	0	NULL	pancreatic cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in the relative risk of pancreatic cancer was similar in former and current snus users and was restricted to current tobacco smokers .
	manualset3
169443	4	410492	13	NULL	NULL	0	NULL	current snus users 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in the relative risk of pancreatic cancer was similar in former and current snus users and was restricted to current tobacco smokers .
	manualset3
169444	5	410492	13	NULL	NULL	0	NULL	tobacco smokers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in the relative risk of pancreatic cancer was similar in former and current snus users and was restricted to current tobacco smokers .
	manualset3
169446	1	410493	13	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase of acid phosphatase activity averaged 63 % .
	manualset3
169447	2	410493	13	NULL	NULL	0	NULL	acid phosphatase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase of acid phosphatase activity averaged 63 % .
	manualset3
169448	3	410493	13	NULL	NULL	0	NULL	63 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase of acid phosphatase activity averaged 63 % .
	manualset3
169449	1	410494	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase of incubation time enhanced propidium iodide uptake by neuroblastoma cells .
	manualset3
169450	2	410494	13	NULL	NULL	0	NULL	incubation time	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase of incubation time enhanced propidium iodide uptake by neuroblastoma cells .
	manualset3
169451	3	410494	13	NULL	NULL	0	NULL	propidium iodide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase of incubation time enhanced propidium iodide uptake by neuroblastoma cells .
	manualset3
169452	4	410494	13	NULL	NULL	0	NULL	uptake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase of incubation time enhanced propidium iodide uptake by neuroblastoma cells .
	manualset3
169453	5	410494	13	NULL	NULL	0	NULL	neuroblastoma cells	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase of incubation time enhanced propidium iodide uptake by neuroblastoma cells .
	manualset3
169469	1	410495	13	NULL	NULL	0	NULL	diffusion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased diffusion in the capillary tumor bed must occur through TNF-independent mechanisms such as intrinsic features of tumor neovasculature , hyperthermia , or other unrecognized perfusion-related factors .
	manualset3
169470	2	410495	13	NULL	NULL	0	NULL	capillary tumor bed	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased diffusion in the capillary tumor bed must occur through TNF-independent mechanisms such as intrinsic features of tumor neovasculature , hyperthermia , or other unrecognized perfusion-related factors .
	manualset3
169471	3	410495	13	NULL	NULL	0	NULL	TNF-independent mechanisms 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased diffusion in the capillary tumor bed must occur through TNF-independent mechanisms such as intrinsic features of tumor neovasculature , hyperthermia , or other unrecognized perfusion-related factors .
	manualset3
169472	4	410495	13	NULL	NULL	0	NULL	intrinsic features 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased diffusion in the capillary tumor bed must occur through TNF-independent mechanisms such as intrinsic features of tumor neovasculature , hyperthermia , or other unrecognized perfusion-related factors .
	manualset3
169473	5	410495	13	NULL	NULL	0	NULL	tumor neovasculature	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased diffusion in the capillary tumor bed must occur through TNF-independent mechanisms such as intrinsic features of tumor neovasculature , hyperthermia , or other unrecognized perfusion-related factors .
	manualset3
169474	6	410495	13	NULL	NULL	0	NULL	hyperthermia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased diffusion in the capillary tumor bed must occur through TNF-independent mechanisms such as intrinsic features of tumor neovasculature , hyperthermia , or other unrecognized perfusion-related factors .
	manualset3
169475	7	410495	13	NULL	NULL	0	NULL	perfusion-related factors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased diffusion in the capillary tumor bed must occur through TNF-independent mechanisms such as intrinsic features of tumor neovasculature , hyperthermia , or other unrecognized perfusion-related factors .
	manualset3
169476	1	410496	13	NULL	NULL	0	NULL	frequency 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased frequency of AA in genetically related individuals , suggests that human AA expression also involves genetic susceptibility .
	manualset3
169477	2	410496	13	NULL	NULL	0	NULL	AA 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased frequency of AA in genetically related individuals , suggests that human AA expression also involves genetic susceptibility .
	manualset3
169478	3	410496	13	NULL	NULL	0	NULL	individuals 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased frequency of AA in genetically related individuals , suggests that human AA expression also involves genetic susceptibility .
	manualset3
169479	4	410496	13	NULL	NULL	0	NULL	human AA expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased frequency of AA in genetically related individuals , suggests that human AA expression also involves genetic susceptibility .
	manualset3
169480	5	410496	13	NULL	NULL	0	NULL	genetic susceptibility 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased frequency of AA in genetically related individuals , suggests that human AA expression also involves genetic susceptibility .
	manualset3
169481	1	410497	13	NULL	NULL	0	NULL	resistance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased resistance of erythrocytes to hemolysis , the increased glutathione peroxidase activity , and the increased degree of unsaturation of fatty acids in the erythrocyte membrane are compatible with a reduction of oxidative stress during hemodialysis with vitamin E-modified membranes .
	manualset3
169482	2	410497	13	NULL	NULL	0	NULL	erythrocytes 	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased resistance of erythrocytes to hemolysis , the increased glutathione peroxidase activity , and the increased degree of unsaturation of fatty acids in the erythrocyte membrane are compatible with a reduction of oxidative stress during hemodialysis with vitamin E-modified membranes .
	manualset3
169483	3	410497	13	NULL	NULL	0	NULL	hemolysis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased resistance of erythrocytes to hemolysis , the increased glutathione peroxidase activity , and the increased degree of unsaturation of fatty acids in the erythrocyte membrane are compatible with a reduction of oxidative stress during hemodialysis with vitamin E-modified membranes .
	manualset3
169484	4	410497	13	NULL	NULL	0	NULL	glutathione peroxidase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased resistance of erythrocytes to hemolysis , the increased glutathione peroxidase activity , and the increased degree of unsaturation of fatty acids in the erythrocyte membrane are compatible with a reduction of oxidative stress during hemodialysis with vitamin E-modified membranes .
	manualset3
169485	5	410497	13	NULL	NULL	0	NULL	degree	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased resistance of erythrocytes to hemolysis , the increased glutathione peroxidase activity , and the increased degree of unsaturation of fatty acids in the erythrocyte membrane are compatible with a reduction of oxidative stress during hemodialysis with vitamin E-modified membranes .
	manualset3
169486	6	410497	13	NULL	NULL	0	NULL	unsaturation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased resistance of erythrocytes to hemolysis , the increased glutathione peroxidase activity , and the increased degree of unsaturation of fatty acids in the erythrocyte membrane are compatible with a reduction of oxidative stress during hemodialysis with vitamin E-modified membranes .
	manualset3
169487	7	410497	13	NULL	NULL	0	NULL	fatty acids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased resistance of erythrocytes to hemolysis , the increased glutathione peroxidase activity , and the increased degree of unsaturation of fatty acids in the erythrocyte membrane are compatible with a reduction of oxidative stress during hemodialysis with vitamin E-modified membranes .
	manualset3
169488	8	410497	13	NULL	NULL	0	NULL	erythrocyte membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased resistance of erythrocytes to hemolysis , the increased glutathione peroxidase activity , and the increased degree of unsaturation of fatty acids in the erythrocyte membrane are compatible with a reduction of oxidative stress during hemodialysis with vitamin E-modified membranes .
	manualset3
169489	9	410497	13	NULL	NULL	0	NULL	reduction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased resistance of erythrocytes to hemolysis , the increased glutathione peroxidase activity , and the increased degree of unsaturation of fatty acids in the erythrocyte membrane are compatible with a reduction of oxidative stress during hemodialysis with vitamin E-modified membranes .
	manualset3
169490	10	410497	13	NULL	NULL	0	NULL	oxidative stress	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased resistance of erythrocytes to hemolysis , the increased glutathione peroxidase activity , and the increased degree of unsaturation of fatty acids in the erythrocyte membrane are compatible with a reduction of oxidative stress during hemodialysis with vitamin E-modified membranes .
	manualset3
169491	11	410497	13	NULL	NULL	0	NULL	hemodialysis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased resistance of erythrocytes to hemolysis , the increased glutathione peroxidase activity , and the increased degree of unsaturation of fatty acids in the erythrocyte membrane are compatible with a reduction of oxidative stress during hemodialysis with vitamin E-modified membranes .
	manualset3
169492	12	410497	13	NULL	NULL	0	NULL	vitamin E-modified membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased resistance of erythrocytes to hemolysis , the increased glutathione peroxidase activity , and the increased degree of unsaturation of fatty acids in the erythrocyte membrane are compatible with a reduction of oxidative stress during hemodialysis with vitamin E-modified membranes .
	manualset3
169493	1	410498	13	NULL	NULL	0	NULL	increases 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The increases in plasma prolactin concentrations which have been demonstrated in previous studies in response to osmotic stress are strongly suggestive of a role for prolactin in avian osmoregulation .
	manualset3
169494	2	410498	13	NULL	NULL	0	NULL	plasma prolactin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The increases in plasma prolactin concentrations which have been demonstrated in previous studies in response to osmotic stress are strongly suggestive of a role for prolactin in avian osmoregulation .
	manualset3
169495	3	410498	13	NULL	NULL	0	NULL	concentrations 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The increases in plasma prolactin concentrations which have been demonstrated in previous studies in response to osmotic stress are strongly suggestive of a role for prolactin in avian osmoregulation .
	manualset3
169496	4	410498	13	NULL	NULL	0	NULL	previous studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The increases in plasma prolactin concentrations which have been demonstrated in previous studies in response to osmotic stress are strongly suggestive of a role for prolactin in avian osmoregulation .
	manualset3
169497	5	410498	13	NULL	NULL	0	NULL	response	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The increases in plasma prolactin concentrations which have been demonstrated in previous studies in response to osmotic stress are strongly suggestive of a role for prolactin in avian osmoregulation .
	manualset3
169498	6	410498	13	NULL	NULL	0	NULL	osmotic stress 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The increases in plasma prolactin concentrations which have been demonstrated in previous studies in response to osmotic stress are strongly suggestive of a role for prolactin in avian osmoregulation .
	manualset3
169499	7	410498	13	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The increases in plasma prolactin concentrations which have been demonstrated in previous studies in response to osmotic stress are strongly suggestive of a role for prolactin in avian osmoregulation .
	manualset3
169500	8	410498	13	NULL	NULL	0	NULL	prolactin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The increases in plasma prolactin concentrations which have been demonstrated in previous studies in response to osmotic stress are strongly suggestive of a role for prolactin in avian osmoregulation .
	manualset3
169501	9	410498	13	NULL	NULL	0	NULL	avian osmoregulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The increases in plasma prolactin concentrations which have been demonstrated in previous studies in response to osmotic stress are strongly suggestive of a role for prolactin in avian osmoregulation .
	manualset3
169502	1	410499	13	NULL	NULL	0	NULL	rank order	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The increasing rank order for effectiveness , with doses in milligrams , was placebo , P50 , aspirin 650 , F600 , F50 , P50 + F50 , F200 , P50 + F600 , P50 + F200 , P200 + F50 , P200 , P200 + F200 , and P200 + F600 .
	manualset3
169503	2	410499	13	NULL	NULL	0	NULL	effectiveness 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The increasing rank order for effectiveness , with doses in milligrams , was placebo , P50 , aspirin 650 , F600 , F50 , P50 + F50 , F200 , P50 + F600 , P50 + F200 , P200 + F50 , P200 , P200 + F200 , and P200 + F600 .
	manualset3
169504	3	410499	13	NULL	NULL	0	NULL	doses 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The increasing rank order for effectiveness , with doses in milligrams , was placebo , P50 , aspirin 650 , F600 , F50 , P50 + F50 , F200 , P50 + F600 , P50 + F200 , P200 + F50 , P200 , P200 + F200 , and P200 + F600 .
	manualset3
169505	4	410499	13	NULL	NULL	0	NULL	milligrams 	Unit												NULL		0	NULL	NULL	NULL	NULL	NULL	The increasing rank order for effectiveness , with doses in milligrams , was placebo , P50 , aspirin 650 , F600 , F50 , P50 + F50 , F200 , P50 + F600 , P50 + F200 , P200 + F50 , P200 , P200 + F200 , and P200 + F600 .
	manualset3
169506	5	410499	13	NULL	NULL	0	NULL	placebo	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The increasing rank order for effectiveness , with doses in milligrams , was placebo , P50 , aspirin 650 , F600 , F50 , P50 + F50 , F200 , P50 + F600 , P50 + F200 , P200 + F50 , P200 , P200 + F200 , and P200 + F600 .
	manualset3
169507	6	410499	13	NULL	NULL	0	NULL	P50 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The increasing rank order for effectiveness , with doses in milligrams , was placebo , P50 , aspirin 650 , F600 , F50 , P50 + F50 , F200 , P50 + F600 , P50 + F200 , P200 + F50 , P200 , P200 + F200 , and P200 + F600 .
	manualset3
169508	7	410499	13	NULL	NULL	0	NULL	aspirin 650	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The increasing rank order for effectiveness , with doses in milligrams , was placebo , P50 , aspirin 650 , F600 , F50 , P50 + F50 , F200 , P50 + F600 , P50 + F200 , P200 + F50 , P200 , P200 + F200 , and P200 + F600 .
	manualset3
169509	8	410499	13	NULL	NULL	0	NULL	F600 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The increasing rank order for effectiveness , with doses in milligrams , was placebo , P50 , aspirin 650 , F600 , F50 , P50 + F50 , F200 , P50 + F600 , P50 + F200 , P200 + F50 , P200 , P200 + F200 , and P200 + F600 .
	manualset3
169510	9	410499	13	NULL	NULL	0	NULL	F50 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The increasing rank order for effectiveness , with doses in milligrams , was placebo , P50 , aspirin 650 , F600 , F50 , P50 + F50 , F200 , P50 + F600 , P50 + F200 , P200 + F50 , P200 , P200 + F200 , and P200 + F600 .
	manualset3
169511	10	410499	13	NULL	NULL	0	NULL	P50 + F50	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The increasing rank order for effectiveness , with doses in milligrams , was placebo , P50 , aspirin 650 , F600 , F50 , P50 + F50 , F200 , P50 + F600 , P50 + F200 , P200 + F50 , P200 , P200 + F200 , and P200 + F600 .
	manualset3
169512	11	410499	13	NULL	NULL	0	NULL	F200 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The increasing rank order for effectiveness , with doses in milligrams , was placebo , P50 , aspirin 650 , F600 , F50 , P50 + F50 , F200 , P50 + F600 , P50 + F200 , P200 + F50 , P200 , P200 + F200 , and P200 + F600 .
	manualset3
169513	12	410499	13	NULL	NULL	0	NULL	P50 + F600 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The increasing rank order for effectiveness , with doses in milligrams , was placebo , P50 , aspirin 650 , F600 , F50 , P50 + F50 , F200 , P50 + F600 , P50 + F200 , P200 + F50 , P200 , P200 + F200 , and P200 + F600 .
	manualset3
169514	1	410500	13	NULL	NULL	0	NULL	incremental CE ratio ( ICER ) 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The incremental CE ratio ( ICER ) to find the CA missed by RAD was $ 66608 per CA .
	manualset3
169515	2	410500	13	NULL	NULL	0	NULL	CA 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The incremental CE ratio ( ICER ) to find the CA missed by RAD was $ 66608 per CA .
	manualset3
169516	3	410500	13	NULL	NULL	0	NULL	RAD	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The incremental CE ratio ( ICER ) to find the CA missed by RAD was $ 66608 per CA .
	manualset3
169517	4	410500	13	NULL	NULL	0	NULL	$ 66608 per CA	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The incremental CE ratio ( ICER ) to find the CA missed by RAD was $ 66608 per CA .
	manualset3
169518	1	410501	13	NULL	NULL	0	NULL	indexes	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The indexes required that binding be negligible compared to the efflux of labeled NMSP ( i.e. , k2 much greater than k3 ) and therefore yielded incorrectly low values of k3 .
	manualset3
169519	2	410501	13	NULL	NULL	0	NULL	binding 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The indexes required that binding be negligible compared to the efflux of labeled NMSP ( i.e. , k2 much greater than k3 ) and therefore yielded incorrectly low values of k3 .
	manualset3
169520	3	410501	13	NULL	NULL	0	NULL	efflux 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The indexes required that binding be negligible compared to the efflux of labeled NMSP ( i.e. , k2 much greater than k3 ) and therefore yielded incorrectly low values of k3 .
	manualset3
169521	4	410501	13	NULL	NULL	0	NULL	NMSP 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The indexes required that binding be negligible compared to the efflux of labeled NMSP ( i.e. , k2 much greater than k3 ) and therefore yielded incorrectly low values of k3 .
	manualset3
169522	5	410501	13	NULL	NULL	0	NULL	k2 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The indexes required that binding be negligible compared to the efflux of labeled NMSP ( i.e. , k2 much greater than k3 ) and therefore yielded incorrectly low values of k3 .
	manualset3
169523	6	410501	13	NULL	NULL	0	NULL	k3 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The indexes required that binding be negligible compared to the efflux of labeled NMSP ( i.e. , k2 much greater than k3 ) and therefore yielded incorrectly low values of k3 .
	manualset3
169524	7	410501	13	NULL	NULL	0	NULL	low values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The indexes required that binding be negligible compared to the efflux of labeled NMSP ( i.e. , k2 much greater than k3 ) and therefore yielded incorrectly low values of k3 .
	manualset3
169525	8	410501	13	NULL	NULL	0	NULL	k3 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The indexes required that binding be negligible compared to the efflux of labeled NMSP ( i.e. , k2 much greater than k3 ) and therefore yielded incorrectly low values of k3 .
	manualset3
169526	1	410502	13	NULL	NULL	0	NULL	indication 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The indication for surgical operation was established : Small bowel enteroclysis revealed an oval filling defect in the lumen of ileum .
	manualset3
169527	2	410502	13	NULL	NULL	0	NULL	surgical operation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The indication for surgical operation was established : Small bowel enteroclysis revealed an oval filling defect in the lumen of ileum .
	manualset3
169528	2	410502	13	NULL	NULL	0	NULL	surgical operation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The indication for surgical operation was established : Small bowel enteroclysis revealed an oval filling defect in the lumen of ileum .
	manualset3
169529	2	410502	13	NULL	NULL	0	NULL	surgical operation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The indication for surgical operation was established : Small bowel enteroclysis revealed an oval filling defect in the lumen of ileum .
	manualset3
169530	3	410502	13	NULL	NULL	0	NULL	Small bowel enteroclysis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The indication for surgical operation was established : Small bowel enteroclysis revealed an oval filling defect in the lumen of ileum .
	manualset3
169531	4	410502	13	NULL	NULL	0	NULL	oval filling defect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The indication for surgical operation was established : Small bowel enteroclysis revealed an oval filling defect in the lumen of ileum .
	manualset3
169532	5	410502	13	NULL	NULL	0	NULL	lumen of ileum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The indication for surgical operation was established : Small bowel enteroclysis revealed an oval filling defect in the lumen of ileum .
	manualset3
169533	1	410503	13	NULL	NULL	0	NULL	indications 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The indications are significant instability and severe pain relieved by immobilization .
	manualset3
169534	2	410503	13	NULL	NULL	0	NULL	instability 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The indications are significant instability and severe pain relieved by immobilization .
	manualset3
169535	3	410503	13	NULL	NULL	0	NULL	severe pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The indications are significant instability and severe pain relieved by immobilization .
	manualset3
169536	4	410503	13	NULL	NULL	NULL	NULL	immobilization 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The indications are significant instability and severe pain relieved by immobilization .
	manualset3
169537	1	410504	13	NULL	NULL	0	NULL	total 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 1096 men and 580 women aged 30 to 69 years and with body mass index of 18.5 to 29.9 kg/m ( 2 ) were recruited .
	manualset3
169538	2	410504	13	NULL	NULL	0	NULL	1096 men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 1096 men and 580 women aged 30 to 69 years and with body mass index of 18.5 to 29.9 kg/m ( 2 ) were recruited .
	manualset3
169539	3	410504	13	NULL	NULL	0	NULL	580 women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 1096 men and 580 women aged 30 to 69 years and with body mass index of 18.5 to 29.9 kg/m ( 2 ) were recruited .
	manualset3
169540	4	410504	13	NULL	NULL	0	NULL	30 to 69 years 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 1096 men and 580 women aged 30 to 69 years and with body mass index of 18.5 to 29.9 kg/m ( 2 ) were recruited .
	manualset3
169541	5	410504	13	NULL	NULL	0	NULL	body mass index	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 1096 men and 580 women aged 30 to 69 years and with body mass index of 18.5 to 29.9 kg/m ( 2 ) were recruited .
	manualset3
169542	6	410504	13	NULL	NULL	0	NULL	18.5 to 29.9 kg/m	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 1096 men and 580 women aged 30 to 69 years and with body mass index of 18.5 to 29.9 kg/m ( 2 ) were recruited .
	manualset3
169543	1	410505	13	NULL	NULL	0	NULL	indications 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The indications for urgent revascularization of the myocardium in cases of infarction included the inefficacy of drug therapy within 2-3 hours of its onset , an unarrested pulmonary oedema and cardiogenic shock in cases of localized proximal occlusion of the coronaries revealed by elective or urgent coronary angiography .
	manualset3
169544	2	410505	13	NULL	NULL	0	NULL	revascularization 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The indications for urgent revascularization of the myocardium in cases of infarction included the inefficacy of drug therapy within 2-3 hours of its onset , an unarrested pulmonary oedema and cardiogenic shock in cases of localized proximal occlusion of the coronaries revealed by elective or urgent coronary angiography .
	manualset3
169545	3	410505	13	NULL	NULL	0	NULL	myocardium 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The indications for urgent revascularization of the myocardium in cases of infarction included the inefficacy of drug therapy within 2-3 hours of its onset , an unarrested pulmonary oedema and cardiogenic shock in cases of localized proximal occlusion of the coronaries revealed by elective or urgent coronary angiography .
	manualset3
169546	4	410505	13	NULL	NULL	0	NULL	cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The indications for urgent revascularization of the myocardium in cases of infarction included the inefficacy of drug therapy within 2-3 hours of its onset , an unarrested pulmonary oedema and cardiogenic shock in cases of localized proximal occlusion of the coronaries revealed by elective or urgent coronary angiography .
	manualset3
169547	5	410505	13	NULL	NULL	0	NULL	infarction 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The indications for urgent revascularization of the myocardium in cases of infarction included the inefficacy of drug therapy within 2-3 hours of its onset , an unarrested pulmonary oedema and cardiogenic shock in cases of localized proximal occlusion of the coronaries revealed by elective or urgent coronary angiography .
	manualset3
169548	6	410505	13	NULL	NULL	0	NULL	inefficacy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The indications for urgent revascularization of the myocardium in cases of infarction included the inefficacy of drug therapy within 2-3 hours of its onset , an unarrested pulmonary oedema and cardiogenic shock in cases of localized proximal occlusion of the coronaries revealed by elective or urgent coronary angiography .
	manualset3
169549	7	410505	13	NULL	NULL	0	NULL	drug therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The indications for urgent revascularization of the myocardium in cases of infarction included the inefficacy of drug therapy within 2-3 hours of its onset , an unarrested pulmonary oedema and cardiogenic shock in cases of localized proximal occlusion of the coronaries revealed by elective or urgent coronary angiography .
	manualset3
169550	8	410505	13	NULL	NULL	0	NULL	2-3 hours 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The indications for urgent revascularization of the myocardium in cases of infarction included the inefficacy of drug therapy within 2-3 hours of its onset , an unarrested pulmonary oedema and cardiogenic shock in cases of localized proximal occlusion of the coronaries revealed by elective or urgent coronary angiography .
	manualset3
169551	9	410505	13	NULL	NULL	0	NULL	onset 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The indications for urgent revascularization of the myocardium in cases of infarction included the inefficacy of drug therapy within 2-3 hours of its onset , an unarrested pulmonary oedema and cardiogenic shock in cases of localized proximal occlusion of the coronaries revealed by elective or urgent coronary angiography .
	manualset3
169552	10	410505	13	NULL	NULL	0	NULL	pulmonary oedema	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The indications for urgent revascularization of the myocardium in cases of infarction included the inefficacy of drug therapy within 2-3 hours of its onset , an unarrested pulmonary oedema and cardiogenic shock in cases of localized proximal occlusion of the coronaries revealed by elective or urgent coronary angiography .
	manualset3
169553	11	410505	13	NULL	NULL	0	NULL	cardiogenic shock	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The indications for urgent revascularization of the myocardium in cases of infarction included the inefficacy of drug therapy within 2-3 hours of its onset , an unarrested pulmonary oedema and cardiogenic shock in cases of localized proximal occlusion of the coronaries revealed by elective or urgent coronary angiography .
	manualset3
169554	12	410505	13	NULL	NULL	0	NULL	cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The indications for urgent revascularization of the myocardium in cases of infarction included the inefficacy of drug therapy within 2-3 hours of its onset , an unarrested pulmonary oedema and cardiogenic shock in cases of localized proximal occlusion of the coronaries revealed by elective or urgent coronary angiography .
	manualset3
169555	13	410505	13	NULL	NULL	0	NULL	localized proximal occlusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The indications for urgent revascularization of the myocardium in cases of infarction included the inefficacy of drug therapy within 2-3 hours of its onset , an unarrested pulmonary oedema and cardiogenic shock in cases of localized proximal occlusion of the coronaries revealed by elective or urgent coronary angiography .
	manualset3
169556	14	410505	13	NULL	NULL	0	NULL	coronaries 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The indications for urgent revascularization of the myocardium in cases of infarction included the inefficacy of drug therapy within 2-3 hours of its onset , an unarrested pulmonary oedema and cardiogenic shock in cases of localized proximal occlusion of the coronaries revealed by elective or urgent coronary angiography .
	manualset3
169557	15	410505	13	NULL	NULL	NULL	NULL	elective coronary angiography	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The indications for urgent revascularization of the myocardium in cases of infarction included the inefficacy of drug therapy within 2-3 hours of its onset , an unarrested pulmonary oedema and cardiogenic shock in cases of localized proximal occlusion of the coronaries revealed by elective or urgent coronary angiography .
	manualset3
178666	16	410505	13	NULL	NULL	0	NULL	urgent coronary angiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The indications for urgent revascularization of the myocardium in cases of infarction included the inefficacy of drug therapy within 2-3 hours of its onset , an unarrested pulmonary oedema and cardiogenic shock in cases of localized proximal occlusion of the coronaries revealed by elective or urgent coronary angiography .
	manualset3
169558	1	410506	13	NULL	NULL	0	NULL	indices 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The indices included in this analysis were hepatic blood flow ( Q ) and maximal receptor binding rate ( Rmax ) , which showed a good correlation with semiquantitative ratio indices for 99mTc-GSA , namely the retention rate in blood ( HH15 ) and the hepatic uptake rate ( LHL15 ) .
	manualset3
169559	2	410506	13	NULL	NULL	0	NULL	analysis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The indices included in this analysis were hepatic blood flow ( Q ) and maximal receptor binding rate ( Rmax ) , which showed a good correlation with semiquantitative ratio indices for 99mTc-GSA , namely the retention rate in blood ( HH15 ) and the hepatic uptake rate ( LHL15 ) .
	manualset3
169560	3	410506	13	NULL	NULL	0	NULL	hepatic blood flow ( Q )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The indices included in this analysis were hepatic blood flow ( Q ) and maximal receptor binding rate ( Rmax ) , which showed a good correlation with semiquantitative ratio indices for 99mTc-GSA , namely the retention rate in blood ( HH15 ) and the hepatic uptake rate ( LHL15 ) .
	manualset3
169561	4	410506	13	NULL	NULL	0	NULL	maximal receptor binding rate ( Rmax ) 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The indices included in this analysis were hepatic blood flow ( Q ) and maximal receptor binding rate ( Rmax ) , which showed a good correlation with semiquantitative ratio indices for 99mTc-GSA , namely the retention rate in blood ( HH15 ) and the hepatic uptake rate ( LHL15 ) .
	manualset3
169562	5	410506	13	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The indices included in this analysis were hepatic blood flow ( Q ) and maximal receptor binding rate ( Rmax ) , which showed a good correlation with semiquantitative ratio indices for 99mTc-GSA , namely the retention rate in blood ( HH15 ) and the hepatic uptake rate ( LHL15 ) .
	manualset3
169563	6	410506	13	NULL	NULL	0	NULL	semiquantitative ratio indices	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The indices included in this analysis were hepatic blood flow ( Q ) and maximal receptor binding rate ( Rmax ) , which showed a good correlation with semiquantitative ratio indices for 99mTc-GSA , namely the retention rate in blood ( HH15 ) and the hepatic uptake rate ( LHL15 ) .
	manualset3
169564	7	410506	13	NULL	NULL	0	NULL	99mTc-GSA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The indices included in this analysis were hepatic blood flow ( Q ) and maximal receptor binding rate ( Rmax ) , which showed a good correlation with semiquantitative ratio indices for 99mTc-GSA , namely the retention rate in blood ( HH15 ) and the hepatic uptake rate ( LHL15 ) .
	manualset3
169565	8	410506	13	NULL	NULL	0	NULL	retention rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The indices included in this analysis were hepatic blood flow ( Q ) and maximal receptor binding rate ( Rmax ) , which showed a good correlation with semiquantitative ratio indices for 99mTc-GSA , namely the retention rate in blood ( HH15 ) and the hepatic uptake rate ( LHL15 ) .
	manualset3
169566	9	410506	13	NULL	NULL	0	NULL	blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The indices included in this analysis were hepatic blood flow ( Q ) and maximal receptor binding rate ( Rmax ) , which showed a good correlation with semiquantitative ratio indices for 99mTc-GSA , namely the retention rate in blood ( HH15 ) and the hepatic uptake rate ( LHL15 ) .
	manualset3
169567	10	410506	13	NULL	NULL	0	NULL	HH15	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The indices included in this analysis were hepatic blood flow ( Q ) and maximal receptor binding rate ( Rmax ) , which showed a good correlation with semiquantitative ratio indices for 99mTc-GSA , namely the retention rate in blood ( HH15 ) and the hepatic uptake rate ( LHL15 ) .
	manualset3
169568	11	410506	13	NULL	NULL	0	NULL	hepatic uptake rate ( LHL15 )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The indices included in this analysis were hepatic blood flow ( Q ) and maximal receptor binding rate ( Rmax ) , which showed a good correlation with semiquantitative ratio indices for 99mTc-GSA , namely the retention rate in blood ( HH15 ) and the hepatic uptake rate ( LHL15 ) .
	manualset3
169569	1	410507	13	NULL	NULL	0	NULL	indices 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The indices of burn traumatism in the Dnepropetrovsk region for the 10-year period are presented , and lethality in burns at the regional burn department is analyzed .
	manualset3
169570	2	410507	13	NULL	NULL	0	NULL	burn traumatism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The indices of burn traumatism in the Dnepropetrovsk region for the 10-year period are presented , and lethality in burns at the regional burn department is analyzed .
	manualset3
169571	3	410507	13	NULL	NULL	0	NULL	Dnepropetrovsk region	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The indices of burn traumatism in the Dnepropetrovsk region for the 10-year period are presented , and lethality in burns at the regional burn department is analyzed .
	manualset3
169572	4	410507	13	NULL	NULL	0	NULL	10-year period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The indices of burn traumatism in the Dnepropetrovsk region for the 10-year period are presented , and lethality in burns at the regional burn department is analyzed .
	manualset3
169573	5	410507	13	NULL	NULL	0	NULL	lethality 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The indices of burn traumatism in the Dnepropetrovsk region for the 10-year period are presented , and lethality in burns at the regional burn department is analyzed .
	manualset3
169574	6	410507	13	NULL	NULL	0	NULL	burns	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The indices of burn traumatism in the Dnepropetrovsk region for the 10-year period are presented , and lethality in burns at the regional burn department is analyzed .
	manualset3
169575	7	410507	13	NULL	NULL	0	NULL	regional burn department 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The indices of burn traumatism in the Dnepropetrovsk region for the 10-year period are presented , and lethality in burns at the regional burn department is analyzed .
	manualset3
169576	1	410508	13	NULL	NULL	0	NULL	indices 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The indices of immune status , concentration of alpha 1-thymosin and level of thymus epithelial cell autoantibodies in human blood of persons , who had worked in 30-km zone Chernobyl NPP were studied .
	manualset3
169577	2	410508	13	NULL	NULL	0	NULL	immune status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The indices of immune status , concentration of alpha 1-thymosin and level of thymus epithelial cell autoantibodies in human blood of persons , who had worked in 30-km zone Chernobyl NPP were studied .
	manualset3
169578	3	410508	13	NULL	NULL	0	NULL	concentration 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The indices of immune status , concentration of alpha 1-thymosin and level of thymus epithelial cell autoantibodies in human blood of persons , who had worked in 30-km zone Chernobyl NPP were studied .
	manualset3
169579	4	410508	13	NULL	NULL	0	NULL	alpha 1-thymosin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The indices of immune status , concentration of alpha 1-thymosin and level of thymus epithelial cell autoantibodies in human blood of persons , who had worked in 30-km zone Chernobyl NPP were studied .
	manualset3
169580	5	410508	13	NULL	NULL	0	NULL	level	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The indices of immune status , concentration of alpha 1-thymosin and level of thymus epithelial cell autoantibodies in human blood of persons , who had worked in 30-km zone Chernobyl NPP were studied .
	manualset3
169581	6	410508	13	NULL	NULL	0	NULL	thymus epithelial cell autoantibodies 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The indices of immune status , concentration of alpha 1-thymosin and level of thymus epithelial cell autoantibodies in human blood of persons , who had worked in 30-km zone Chernobyl NPP were studied .
	manualset3
169582	7	410508	13	NULL	NULL	0	NULL	human blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The indices of immune status , concentration of alpha 1-thymosin and level of thymus epithelial cell autoantibodies in human blood of persons , who had worked in 30-km zone Chernobyl NPP were studied .
	manualset3
169583	8	410508	13	NULL	NULL	0	NULL	persons 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The indices of immune status , concentration of alpha 1-thymosin and level of thymus epithelial cell autoantibodies in human blood of persons , who had worked in 30-km zone Chernobyl NPP were studied .
	manualset3
169584	9	410508	13	NULL	NULL	0	NULL	30-km zone 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The indices of immune status , concentration of alpha 1-thymosin and level of thymus epithelial cell autoantibodies in human blood of persons , who had worked in 30-km zone Chernobyl NPP were studied .
	manualset3
169585	10	410508	13	NULL	NULL	0	NULL	Chernobyl NPP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The indices of immune status , concentration of alpha 1-thymosin and level of thymus epithelial cell autoantibodies in human blood of persons , who had worked in 30-km zone Chernobyl NPP were studied .
	manualset3
169586	1	410509	13	NULL	NULL	0	NULL	hemaglutination test	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The indirect hemaglutination test for melioidosis was studied in 295 children who live in the northeastern part of Thailand .
	manualset3
169587	2	410509	13	NULL	NULL	0	NULL	melioidosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The indirect hemaglutination test for melioidosis was studied in 295 children who live in the northeastern part of Thailand .
	manualset3
169588	3	410509	13	NULL	NULL	0	NULL	295 children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The indirect hemaglutination test for melioidosis was studied in 295 children who live in the northeastern part of Thailand .
	manualset3
169590	4	410509	13	NULL	NULL	0	NULL	northeastern part of Thailand	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The indirect hemaglutination test for melioidosis was studied in 295 children who live in the northeastern part of Thailand .
	manualset3
169591	1	410510	13	NULL	NULL	0	NULL	revascularization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The indirect revascularization of the corpora cavernosa appears to be an acceptable surgical treatment of vasculogenic impotence .
	manualset3
169592	2	410510	13	NULL	NULL	0	NULL	corpora cavernosa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The indirect revascularization of the corpora cavernosa appears to be an acceptable surgical treatment of vasculogenic impotence .
	manualset3
169593	3	410510	13	NULL	NULL	0	NULL	surgical treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The indirect revascularization of the corpora cavernosa appears to be an acceptable surgical treatment of vasculogenic impotence .
	manualset3
169594	4	410510	13	NULL	NULL	0	NULL	vasculogenic impotence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The indirect revascularization of the corpora cavernosa appears to be an acceptable surgical treatment of vasculogenic impotence .
	manualset3
169595	1	410511	13	NULL	NULL	0	NULL	upregulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The indirect upregulation of CTGF expression by Dll1 is likely due to the ability of Dll1icd to increase Wnt signaling , a pathway that targets CTGF .
	manualset3
169596	2	410511	13	NULL	NULL	0	NULL	CTGF expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The indirect upregulation of CTGF expression by Dll1 is likely due to the ability of Dll1icd to increase Wnt signaling , a pathway that targets CTGF .
	manualset3
169597	3	410511	13	NULL	NULL	0	NULL	Dll1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The indirect upregulation of CTGF expression by Dll1 is likely due to the ability of Dll1icd to increase Wnt signaling , a pathway that targets CTGF .
	manualset3
169598	4	410511	13	NULL	NULL	0	NULL	Dll1icd 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The indirect upregulation of CTGF expression by Dll1 is likely due to the ability of Dll1icd to increase Wnt signaling , a pathway that targets CTGF .
	manualset3
169599	5	410511	13	NULL	NULL	0	NULL	Wnt signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The indirect upregulation of CTGF expression by Dll1 is likely due to the ability of Dll1icd to increase Wnt signaling , a pathway that targets CTGF .
	manualset3
169600	6	410511	13	NULL	NULL	0	NULL	pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The indirect upregulation of CTGF expression by Dll1 is likely due to the ability of Dll1icd to increase Wnt signaling , a pathway that targets CTGF .
	manualset3
169601	7	410511	13	NULL	NULL	0	NULL	CTGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The indirect upregulation of CTGF expression by Dll1 is likely due to the ability of Dll1icd to increase Wnt signaling , a pathway that targets CTGF .
	manualset3
169602	8	410511	13	NULL	NULL	0	NULL	ability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The indirect upregulation of CTGF expression by Dll1 is likely due to the ability of Dll1icd to increase Wnt signaling , a pathway that targets CTGF .
	manualset3
169603	9	410511	13	NULL	NULL	0	NULL	targets 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The indirect upregulation of CTGF expression by Dll1 is likely due to the ability of Dll1icd to increase Wnt signaling , a pathway that targets CTGF .
	manualset3
169606	1	410512	13	NULL	NULL	0	NULL	individual TFIIIB subunits	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The individual TFIIIB subunits are nuclear by immunofluorescence and are calculated to have nuclear concentrations in the low micromolar range .
	manualset3
169608	3	410512	13	NULL	NULL	0	NULL	immunofluorescence 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The individual TFIIIB subunits are nuclear by immunofluorescence and are calculated to have nuclear concentrations in the low micromolar range .
	manualset3
169609	4	410512	13	NULL	NULL	NULL	NULL	nuclear concentrations 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The individual TFIIIB subunits are nuclear by immunofluorescence and are calculated to have nuclear concentrations in the low micromolar range .
	manualset3
169610	5	410512	13	NULL	NULL	0	NULL	low micromolar range	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The individual TFIIIB subunits are nuclear by immunofluorescence and are calculated to have nuclear concentrations in the low micromolar range .
	manualset3
169611	1	410513	13	NULL	NULL	NULL	NULL	right	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The individual 's right to refuse treatment may not be subordinated to the state 's interest in protecting the potential life of the fetus .
	manualset3
169612	2	410513	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The individual 's right to refuse treatment may not be subordinated to the state 's interest in protecting the potential life of the fetus .
	manualset3
169613	3	410513	13	NULL	NULL	0	NULL	interest	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The individual 's right to refuse treatment may not be subordinated to the state 's interest in protecting the potential life of the fetus .
	manualset3
169614	4	410513	13	NULL	NULL	0	NULL	potential life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The individual 's right to refuse treatment may not be subordinated to the state 's interest in protecting the potential life of the fetus .
	manualset3
169615	5	410513	13	NULL	NULL	0	NULL	fetus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The individual 's right to refuse treatment may not be subordinated to the state 's interest in protecting the potential life of the fetus .
	manualset3
169616	1	410514	13	NULL	NULL	0	NULL	indomethacin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The indomethacin pretreatment had no effect on pupil size of any group , but phenoxybenzamine ( PBA ) reduced the mydriatic effect , implying a direct or a predominant role of NE on iris muscle .
	manualset3
169617	2	410514	13	NULL	NULL	0	NULL	pretreatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The indomethacin pretreatment had no effect on pupil size of any group , but phenoxybenzamine ( PBA ) reduced the mydriatic effect , implying a direct or a predominant role of NE on iris muscle .
	manualset3
169618	3	410514	13	NULL	NULL	0	NULL	effect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The indomethacin pretreatment had no effect on pupil size of any group , but phenoxybenzamine ( PBA ) reduced the mydriatic effect , implying a direct or a predominant role of NE on iris muscle .
	manualset3
169619	4	410514	13	NULL	NULL	0	NULL	pupil size	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The indomethacin pretreatment had no effect on pupil size of any group , but phenoxybenzamine ( PBA ) reduced the mydriatic effect , implying a direct or a predominant role of NE on iris muscle .
	manualset3
169620	5	410514	13	NULL	NULL	0	NULL	group 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The indomethacin pretreatment had no effect on pupil size of any group , but phenoxybenzamine ( PBA ) reduced the mydriatic effect , implying a direct or a predominant role of NE on iris muscle .
	manualset3
169621	6	410514	13	NULL	NULL	0	NULL	phenoxybenzamine ( PBA )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The indomethacin pretreatment had no effect on pupil size of any group , but phenoxybenzamine ( PBA ) reduced the mydriatic effect , implying a direct or a predominant role of NE on iris muscle .
	manualset3
169622	7	410514	13	NULL	NULL	0	NULL	mydriatic effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The indomethacin pretreatment had no effect on pupil size of any group , but phenoxybenzamine ( PBA ) reduced the mydriatic effect , implying a direct or a predominant role of NE on iris muscle .
	manualset3
169623	8	410514	13	NULL	NULL	0	NULL	role 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The indomethacin pretreatment had no effect on pupil size of any group , but phenoxybenzamine ( PBA ) reduced the mydriatic effect , implying a direct or a predominant role of NE on iris muscle .
	manualset3
169624	9	410514	13	NULL	NULL	0	NULL	NE 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The indomethacin pretreatment had no effect on pupil size of any group , but phenoxybenzamine ( PBA ) reduced the mydriatic effect , implying a direct or a predominant role of NE on iris muscle .
	manualset3
169625	10	410514	13	NULL	NULL	0	NULL	iris muscle 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The indomethacin pretreatment had no effect on pupil size of any group , but phenoxybenzamine ( PBA ) reduced the mydriatic effect , implying a direct or a predominant role of NE on iris muscle .
	manualset3
169626	1	410515	13	NULL	NULL	0	NULL	exposure 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The indoor exposure to biological contaminants ( dust mites and fungi ) , history of prematurity , pneumonia , rhinitis and family history of asthma increased the occurence of symptoms suggestive of asthma in young children .
	manualset3
169627	2	410515	13	NULL	NULL	0	NULL	biological contaminants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The indoor exposure to biological contaminants ( dust mites and fungi ) , history of prematurity , pneumonia , rhinitis and family history of asthma increased the occurence of symptoms suggestive of asthma in young children .
	manualset3
169628	3	410515	13	NULL	NULL	0	NULL	dust mites 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The indoor exposure to biological contaminants ( dust mites and fungi ) , history of prematurity , pneumonia , rhinitis and family history of asthma increased the occurence of symptoms suggestive of asthma in young children .
	manualset3
169629	4	410515	13	NULL	NULL	0	NULL	fungi	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The indoor exposure to biological contaminants ( dust mites and fungi ) , history of prematurity , pneumonia , rhinitis and family history of asthma increased the occurence of symptoms suggestive of asthma in young children .
	manualset3
169630	5	410515	13	NULL	NULL	0	NULL	history of prematurity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The indoor exposure to biological contaminants ( dust mites and fungi ) , history of prematurity , pneumonia , rhinitis and family history of asthma increased the occurence of symptoms suggestive of asthma in young children .
	manualset3
169631	6	410515	13	NULL	NULL	0	NULL	pneumonia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The indoor exposure to biological contaminants ( dust mites and fungi ) , history of prematurity , pneumonia , rhinitis and family history of asthma increased the occurence of symptoms suggestive of asthma in young children .
	manualset3
169632	7	410515	13	NULL	NULL	0	NULL	rhinitis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The indoor exposure to biological contaminants ( dust mites and fungi ) , history of prematurity , pneumonia , rhinitis and family history of asthma increased the occurence of symptoms suggestive of asthma in young children .
	manualset3
169633	8	410515	13	NULL	NULL	0	NULL	family history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The indoor exposure to biological contaminants ( dust mites and fungi ) , history of prematurity , pneumonia , rhinitis and family history of asthma increased the occurence of symptoms suggestive of asthma in young children .
	manualset3
169634	9	410515	13	NULL	NULL	0	NULL	asthma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The indoor exposure to biological contaminants ( dust mites and fungi ) , history of prematurity , pneumonia , rhinitis and family history of asthma increased the occurence of symptoms suggestive of asthma in young children .
	manualset3
169635	10	410515	13	NULL	NULL	0	NULL	occurence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The indoor exposure to biological contaminants ( dust mites and fungi ) , history of prematurity , pneumonia , rhinitis and family history of asthma increased the occurence of symptoms suggestive of asthma in young children .
	manualset3
169636	11	410515	13	NULL	NULL	0	NULL	symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The indoor exposure to biological contaminants ( dust mites and fungi ) , history of prematurity , pneumonia , rhinitis and family history of asthma increased the occurence of symptoms suggestive of asthma in young children .
	manualset3
169637	12	410515	13	NULL	NULL	0	NULL	asthma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The indoor exposure to biological contaminants ( dust mites and fungi ) , history of prematurity , pneumonia , rhinitis and family history of asthma increased the occurence of symptoms suggestive of asthma in young children .
	manualset3
169638	13	410515	13	NULL	NULL	0	NULL	young children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The indoor exposure to biological contaminants ( dust mites and fungi ) , history of prematurity , pneumonia , rhinitis and family history of asthma increased the occurence of symptoms suggestive of asthma in young children .
	manualset3
169640	1	410516	13	NULL	NULL	0	NULL	induction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of UPR by indomethacin was observed similarly in other cells including mesangial cells and tubular epithelial cells .
	manualset3
169641	2	410516	13	NULL	NULL	0	NULL	UPR	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of UPR by indomethacin was observed similarly in other cells including mesangial cells and tubular epithelial cells .
	manualset3
169642	3	410516	13	NULL	NULL	0	NULL	indomethacin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of UPR by indomethacin was observed similarly in other cells including mesangial cells and tubular epithelial cells .
	manualset3
169643	4	410516	13	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of UPR by indomethacin was observed similarly in other cells including mesangial cells and tubular epithelial cells .
	manualset3
169644	5	410516	13	NULL	NULL	0	NULL	mesangial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of UPR by indomethacin was observed similarly in other cells including mesangial cells and tubular epithelial cells .
	manualset3
169645	6	410516	13	NULL	NULL	0	NULL	tubular epithelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of UPR by indomethacin was observed similarly in other cells including mesangial cells and tubular epithelial cells .
	manualset3
169646	1	410517	13	NULL	NULL	0	NULL	induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of c-myc and transforming growth factor-beta2 by cerebral ischemia was inhibited by neuronal expression of IkappaBalpha-SR , whereas induction of GFAP by MCAO was reduced by astrocytic expression of IkappaBalpha-SR .
	manualset3
169647	2	410517	13	NULL	NULL	0	NULL	c-myc 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of c-myc and transforming growth factor-beta2 by cerebral ischemia was inhibited by neuronal expression of IkappaBalpha-SR , whereas induction of GFAP by MCAO was reduced by astrocytic expression of IkappaBalpha-SR .
	manualset3
169648	3	410517	13	NULL	NULL	0	NULL	transforming growth factor-beta2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of c-myc and transforming growth factor-beta2 by cerebral ischemia was inhibited by neuronal expression of IkappaBalpha-SR , whereas induction of GFAP by MCAO was reduced by astrocytic expression of IkappaBalpha-SR .
	manualset3
169649	4	410517	13	NULL	NULL	0	NULL	cerebral ischemia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of c-myc and transforming growth factor-beta2 by cerebral ischemia was inhibited by neuronal expression of IkappaBalpha-SR , whereas induction of GFAP by MCAO was reduced by astrocytic expression of IkappaBalpha-SR .
	manualset3
169651	5	410517	13	NULL	NULL	0	NULL	neuronal expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of c-myc and transforming growth factor-beta2 by cerebral ischemia was inhibited by neuronal expression of IkappaBalpha-SR , whereas induction of GFAP by MCAO was reduced by astrocytic expression of IkappaBalpha-SR .
	manualset3
169652	6	410517	13	NULL	NULL	0	NULL	IkappaBalpha-SR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of c-myc and transforming growth factor-beta2 by cerebral ischemia was inhibited by neuronal expression of IkappaBalpha-SR , whereas induction of GFAP by MCAO was reduced by astrocytic expression of IkappaBalpha-SR .
	manualset3
169653	7	410517	13	NULL	NULL	0	NULL	induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of c-myc and transforming growth factor-beta2 by cerebral ischemia was inhibited by neuronal expression of IkappaBalpha-SR , whereas induction of GFAP by MCAO was reduced by astrocytic expression of IkappaBalpha-SR .
	manualset3
169654	8	410517	13	NULL	NULL	0	NULL	GFAP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of c-myc and transforming growth factor-beta2 by cerebral ischemia was inhibited by neuronal expression of IkappaBalpha-SR , whereas induction of GFAP by MCAO was reduced by astrocytic expression of IkappaBalpha-SR .
	manualset3
169655	9	410517	13	NULL	NULL	0	NULL	MCAO	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of c-myc and transforming growth factor-beta2 by cerebral ischemia was inhibited by neuronal expression of IkappaBalpha-SR , whereas induction of GFAP by MCAO was reduced by astrocytic expression of IkappaBalpha-SR .
	manualset3
169656	10	410517	13	NULL	NULL	0	NULL	astrocytic expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of c-myc and transforming growth factor-beta2 by cerebral ischemia was inhibited by neuronal expression of IkappaBalpha-SR , whereas induction of GFAP by MCAO was reduced by astrocytic expression of IkappaBalpha-SR .
	manualset3
169657	11	410517	13	NULL	NULL	0	NULL	IkappaBalpha-SR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of c-myc and transforming growth factor-beta2 by cerebral ischemia was inhibited by neuronal expression of IkappaBalpha-SR , whereas induction of GFAP by MCAO was reduced by astrocytic expression of IkappaBalpha-SR .
	manualset3
169658	1	410518	13	NULL	NULL	0	NULL	induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of cyclin A is also required for S-phase entry , and we now report that distinct effects of mitogens and the actin cytoskeleton on the phosphorylation of CREB and pocket proteins regulate the extent and timing of cyclin A promoter activity , respectively .
	manualset3
169659	2	410518	13	NULL	NULL	0	NULL	cyclin A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of cyclin A is also required for S-phase entry , and we now report that distinct effects of mitogens and the actin cytoskeleton on the phosphorylation of CREB and pocket proteins regulate the extent and timing of cyclin A promoter activity , respectively .
	manualset3
169660	3	410518	13	NULL	NULL	0	NULL	S-phase entry	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of cyclin A is also required for S-phase entry , and we now report that distinct effects of mitogens and the actin cytoskeleton on the phosphorylation of CREB and pocket proteins regulate the extent and timing of cyclin A promoter activity , respectively .
	manualset3
169661	4	410518	13	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of cyclin A is also required for S-phase entry , and we now report that distinct effects of mitogens and the actin cytoskeleton on the phosphorylation of CREB and pocket proteins regulate the extent and timing of cyclin A promoter activity , respectively .
	manualset3
169662	5	410518	13	NULL	NULL	0	NULL	mitogens	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of cyclin A is also required for S-phase entry , and we now report that distinct effects of mitogens and the actin cytoskeleton on the phosphorylation of CREB and pocket proteins regulate the extent and timing of cyclin A promoter activity , respectively .
	manualset3
169663	6	410518	13	NULL	NULL	0	NULL	actin cytoskeleton	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of cyclin A is also required for S-phase entry , and we now report that distinct effects of mitogens and the actin cytoskeleton on the phosphorylation of CREB and pocket proteins regulate the extent and timing of cyclin A promoter activity , respectively .
	manualset3
169664	7	410518	13	NULL	NULL	0	NULL	phosphorylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of cyclin A is also required for S-phase entry , and we now report that distinct effects of mitogens and the actin cytoskeleton on the phosphorylation of CREB and pocket proteins regulate the extent and timing of cyclin A promoter activity , respectively .
	manualset3
169665	8	410518	13	NULL	NULL	0	NULL	CREB	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of cyclin A is also required for S-phase entry , and we now report that distinct effects of mitogens and the actin cytoskeleton on the phosphorylation of CREB and pocket proteins regulate the extent and timing of cyclin A promoter activity , respectively .
	manualset3
169666	9	410518	13	NULL	NULL	0	NULL	pocket proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of cyclin A is also required for S-phase entry , and we now report that distinct effects of mitogens and the actin cytoskeleton on the phosphorylation of CREB and pocket proteins regulate the extent and timing of cyclin A promoter activity , respectively .
	manualset3
169667	10	410518	13	NULL	NULL	0	NULL	extent	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of cyclin A is also required for S-phase entry , and we now report that distinct effects of mitogens and the actin cytoskeleton on the phosphorylation of CREB and pocket proteins regulate the extent and timing of cyclin A promoter activity , respectively .
	manualset3
169668	11	410518	13	NULL	NULL	0	NULL	timing	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of cyclin A is also required for S-phase entry , and we now report that distinct effects of mitogens and the actin cytoskeleton on the phosphorylation of CREB and pocket proteins regulate the extent and timing of cyclin A promoter activity , respectively .
	manualset3
169669	12	410518	13	NULL	NULL	0	NULL	cyclin A promoter activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of cyclin A is also required for S-phase entry , and we now report that distinct effects of mitogens and the actin cytoskeleton on the phosphorylation of CREB and pocket proteins regulate the extent and timing of cyclin A promoter activity , respectively .
	manualset3
169670	1	410519	13	NULL	NULL	0	NULL	induction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of genes encoding adipogenic proteins ( PPAR , SREBP-1c , SCD1 , and FAS ) was also significantly blunted by 50-80 % in OP9 cells overexpressing GX sPLA ( 2 ) .
	manualset3
169671	2	410519	13	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of genes encoding adipogenic proteins ( PPAR , SREBP-1c , SCD1 , and FAS ) was also significantly blunted by 50-80 % in OP9 cells overexpressing GX sPLA ( 2 ) .
	manualset3
169672	3	410519	13	NULL	NULL	0	NULL	adipogenic proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of genes encoding adipogenic proteins ( PPAR , SREBP-1c , SCD1 , and FAS ) was also significantly blunted by 50-80 % in OP9 cells overexpressing GX sPLA ( 2 ) .
	manualset3
169673	4	410519	13	NULL	NULL	0	NULL	PPAR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of genes encoding adipogenic proteins ( PPAR , SREBP-1c , SCD1 , and FAS ) was also significantly blunted by 50-80 % in OP9 cells overexpressing GX sPLA ( 2 ) .
	manualset3
169674	5	410519	13	NULL	NULL	0	NULL	SREBP-1c	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of genes encoding adipogenic proteins ( PPAR , SREBP-1c , SCD1 , and FAS ) was also significantly blunted by 50-80 % in OP9 cells overexpressing GX sPLA ( 2 ) .
	manualset3
169675	6	410519	13	NULL	NULL	0	NULL	SCD1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of genes encoding adipogenic proteins ( PPAR , SREBP-1c , SCD1 , and FAS ) was also significantly blunted by 50-80 % in OP9 cells overexpressing GX sPLA ( 2 ) .
	manualset3
169676	7	410519	13	NULL	NULL	0	NULL	FAS	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of genes encoding adipogenic proteins ( PPAR , SREBP-1c , SCD1 , and FAS ) was also significantly blunted by 50-80 % in OP9 cells overexpressing GX sPLA ( 2 ) .
	manualset3
169677	8	410519	13	NULL	NULL	0	NULL	50-80 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of genes encoding adipogenic proteins ( PPAR , SREBP-1c , SCD1 , and FAS ) was also significantly blunted by 50-80 % in OP9 cells overexpressing GX sPLA ( 2 ) .
	manualset3
169678	9	410519	13	NULL	NULL	0	NULL	OP9 cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of genes encoding adipogenic proteins ( PPAR , SREBP-1c , SCD1 , and FAS ) was also significantly blunted by 50-80 % in OP9 cells overexpressing GX sPLA ( 2 ) .
	manualset3
169679	10	410519	13	NULL	NULL	0	NULL	GX sPLA ( 2 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of genes encoding adipogenic proteins ( PPAR , SREBP-1c , SCD1 , and FAS ) was also significantly blunted by 50-80 % in OP9 cells overexpressing GX sPLA ( 2 ) .
	manualset3
169680	1	410520	13	NULL	NULL	0	NULL	induction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of this enzyme was found to be mediated by specific binding of Hg to the plasma membrane Na ( + ) - K ( + ) - ATPase ( Bmax : 14 nmoles mg-1 protein ; Ka 1.14 x 10 ( 8 ) moles ) and increase in the specific messenger RNA translating 3 beta-hydroxysteroid dehydrogenase .
	manualset3
169681	2	410520	13	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of this enzyme was found to be mediated by specific binding of Hg to the plasma membrane Na ( + ) - K ( + ) - ATPase ( Bmax : 14 nmoles mg-1 protein ; Ka 1.14 x 10 ( 8 ) moles ) and increase in the specific messenger RNA translating 3 beta-hydroxysteroid dehydrogenase .
	manualset3
169682	3	410520	13	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of this enzyme was found to be mediated by specific binding of Hg to the plasma membrane Na ( + ) - K ( + ) - ATPase ( Bmax : 14 nmoles mg-1 protein ; Ka 1.14 x 10 ( 8 ) moles ) and increase in the specific messenger RNA translating 3 beta-hydroxysteroid dehydrogenase .
	manualset3
169683	4	410520	13	NULL	NULL	NULL	NULL	Hg	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The induction of this enzyme was found to be mediated by specific binding of Hg to the plasma membrane Na ( + ) - K ( + ) - ATPase ( Bmax : 14 nmoles mg-1 protein ; Ka 1.14 x 10 ( 8 ) moles ) and increase in the specific messenger RNA translating 3 beta-hydroxysteroid dehydrogenase .
	manualset3
169684	5	410520	13	NULL	NULL	0	NULL	plasma membrane Na ( + ) - K ( + ) - ATPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of this enzyme was found to be mediated by specific binding of Hg to the plasma membrane Na ( + ) - K ( + ) - ATPase ( Bmax : 14 nmoles mg-1 protein ; Ka 1.14 x 10 ( 8 ) moles ) and increase in the specific messenger RNA translating 3 beta-hydroxysteroid dehydrogenase .
	manualset3
169685	6	410520	13	NULL	NULL	0	NULL	Bmax	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of this enzyme was found to be mediated by specific binding of Hg to the plasma membrane Na ( + ) - K ( + ) - ATPase ( Bmax : 14 nmoles mg-1 protein ; Ka 1.14 x 10 ( 8 ) moles ) and increase in the specific messenger RNA translating 3 beta-hydroxysteroid dehydrogenase .
	manualset3
169686	7	410520	13	NULL	NULL	0	NULL	14 nmoles mg-1 protein	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of this enzyme was found to be mediated by specific binding of Hg to the plasma membrane Na ( + ) - K ( + ) - ATPase ( Bmax : 14 nmoles mg-1 protein ; Ka 1.14 x 10 ( 8 ) moles ) and increase in the specific messenger RNA translating 3 beta-hydroxysteroid dehydrogenase .
	manualset3
169687	8	410520	13	NULL	NULL	0	NULL	Ka 1.14 x 10 ( 8 ) moles	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of this enzyme was found to be mediated by specific binding of Hg to the plasma membrane Na ( + ) - K ( + ) - ATPase ( Bmax : 14 nmoles mg-1 protein ; Ka 1.14 x 10 ( 8 ) moles ) and increase in the specific messenger RNA translating 3 beta-hydroxysteroid dehydrogenase .
	manualset3
169688	9	410520	13	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of this enzyme was found to be mediated by specific binding of Hg to the plasma membrane Na ( + ) - K ( + ) - ATPase ( Bmax : 14 nmoles mg-1 protein ; Ka 1.14 x 10 ( 8 ) moles ) and increase in the specific messenger RNA translating 3 beta-hydroxysteroid dehydrogenase .
	manualset3
169689	10	410520	13	NULL	NULL	0	NULL	messenger RNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of this enzyme was found to be mediated by specific binding of Hg to the plasma membrane Na ( + ) - K ( + ) - ATPase ( Bmax : 14 nmoles mg-1 protein ; Ka 1.14 x 10 ( 8 ) moles ) and increase in the specific messenger RNA translating 3 beta-hydroxysteroid dehydrogenase .
	manualset3
169690	11	410520	13	NULL	NULL	0	NULL	3 beta-hydroxysteroid dehydrogenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of this enzyme was found to be mediated by specific binding of Hg to the plasma membrane Na ( + ) - K ( + ) - ATPase ( Bmax : 14 nmoles mg-1 protein ; Ka 1.14 x 10 ( 8 ) moles ) and increase in the specific messenger RNA translating 3 beta-hydroxysteroid dehydrogenase .
	manualset3
169691	1	410521	13	NULL	NULL	0	NULL	infant	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The infant had a simultaneous candida septicemia secondary to colonisation of a central venous line .
	manualset3
169692	2	410521	13	NULL	NULL	0	NULL	candida septicemia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The infant had a simultaneous candida septicemia secondary to colonisation of a central venous line .
	manualset3
169693	3	410521	13	NULL	NULL	0	NULL	colonisation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The infant had a simultaneous candida septicemia secondary to colonisation of a central venous line .
	manualset3
169694	4	410521	13	NULL	NULL	0	NULL	central venous line	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The infant had a simultaneous candida septicemia secondary to colonisation of a central venous line .
	manualset3
169695	1	410522	13	NULL	NULL	0	NULL	infant	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The infant was born to third degree consanguineous marriage .
	manualset3
169696	2	410522	13	NULL	NULL	0	NULL	third degree	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The infant was born to third degree consanguineous marriage .
	manualset3
169697	3	410522	13	NULL	NULL	0	NULL	consanguineous marriage 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The infant was born to third degree consanguineous marriage .
	manualset3
169698	1	410523	13	NULL	NULL	0	NULL	infant	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The infant was started on daily ascorbic acid treatment .
	manualset3
169699	2	410523	13	NULL	NULL	0	NULL	ascorbic acid 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The infant was started on daily ascorbic acid treatment .
	manualset3
169700	3	410523	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The infant was started on daily ascorbic acid treatment .
	manualset3
169701	1	410524	13	NULL	NULL	0	NULL	infarct volume	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The infarct volume measured on computed tomography on days 4 to 7 and the frequency of poor outcome ( Barthel Index score & lt ; 85 ) at 3 months were significantly lower in patients with prior TIA .
	manualset3
169702	2	410524	13	NULL	NULL	0	NULL	computed tomography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The infarct volume measured on computed tomography on days 4 to 7 and the frequency of poor outcome ( Barthel Index score & lt ; 85 ) at 3 months were significantly lower in patients with prior TIA .
	manualset3
169703	3	410524	13	NULL	NULL	0	NULL	days 4 to 7	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The infarct volume measured on computed tomography on days 4 to 7 and the frequency of poor outcome ( Barthel Index score & lt ; 85 ) at 3 months were significantly lower in patients with prior TIA .
	manualset3
169704	4	410524	13	NULL	NULL	0	NULL	frequency	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The infarct volume measured on computed tomography on days 4 to 7 and the frequency of poor outcome ( Barthel Index score & lt ; 85 ) at 3 months were significantly lower in patients with prior TIA .
	manualset3
169705	5	410524	13	NULL	NULL	0	NULL	outcome	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The infarct volume measured on computed tomography on days 4 to 7 and the frequency of poor outcome ( Barthel Index score & lt ; 85 ) at 3 months were significantly lower in patients with prior TIA .
	manualset3
169706	6	410524	13	NULL	NULL	0	NULL	Barthel Index score & lt ; 85	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The infarct volume measured on computed tomography on days 4 to 7 and the frequency of poor outcome ( Barthel Index score & lt ; 85 ) at 3 months were significantly lower in patients with prior TIA .
	manualset3
169707	7	410524	13	NULL	NULL	0	NULL	3 months 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The infarct volume measured on computed tomography on days 4 to 7 and the frequency of poor outcome ( Barthel Index score & lt ; 85 ) at 3 months were significantly lower in patients with prior TIA .
	manualset3
169708	8	410524	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The infarct volume measured on computed tomography on days 4 to 7 and the frequency of poor outcome ( Barthel Index score & lt ; 85 ) at 3 months were significantly lower in patients with prior TIA .
	manualset3
169709	9	410524	13	NULL	NULL	0	NULL	prior TIA	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The infarct volume measured on computed tomography on days 4 to 7 and the frequency of poor outcome ( Barthel Index score & lt ; 85 ) at 3 months were significantly lower in patients with prior TIA .
	manualset3
169710	1	410525	13	NULL	NULL	0	NULL	infiltrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The infiltrate improved after chest physiotherapy , but sputum cultures remained positive .
	manualset3
169711	2	410525	13	NULL	NULL	0	NULL	chest physiotherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The infiltrate improved after chest physiotherapy , but sputum cultures remained positive .
	manualset3
169712	3	410525	13	NULL	NULL	0	NULL	sputum cultures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The infiltrate improved after chest physiotherapy , but sputum cultures remained positive .
	manualset3
169713	1	410526	13	NULL	NULL	0	NULL	inflammatory infiltrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The inflammatory infiltrate consisted mainly of lymphoid cells , including lymphoid blasts , with increased numbers of class II and IL-2-receptor expressing lymphocytes .
	manualset3
169714	2	410526	13	NULL	NULL	0	NULL	lymphoid cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The inflammatory infiltrate consisted mainly of lymphoid cells , including lymphoid blasts , with increased numbers of class II and IL-2-receptor expressing lymphocytes .
	manualset3
169715	3	410526	13	NULL	NULL	0	NULL	lymphoid blasts 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The inflammatory infiltrate consisted mainly of lymphoid cells , including lymphoid blasts , with increased numbers of class II and IL-2-receptor expressing lymphocytes .
	manualset3
169716	4	410526	13	NULL	NULL	0	NULL	numbers 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The inflammatory infiltrate consisted mainly of lymphoid cells , including lymphoid blasts , with increased numbers of class II and IL-2-receptor expressing lymphocytes .
	manualset3
169717	5	410526	13	NULL	NULL	0	NULL	class II	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The inflammatory infiltrate consisted mainly of lymphoid cells , including lymphoid blasts , with increased numbers of class II and IL-2-receptor expressing lymphocytes .
	manualset3
169718	6	410526	13	NULL	NULL	NULL	NULL	IL-2-receptor	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The inflammatory infiltrate consisted mainly of lymphoid cells , including lymphoid blasts , with increased numbers of class II and IL-2-receptor expressing lymphocytes .
	manualset3
169719	7	410526	13	NULL	NULL	0	NULL	lymphocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The inflammatory infiltrate consisted mainly of lymphoid cells , including lymphoid blasts , with increased numbers of class II and IL-2-receptor expressing lymphocytes .
	manualset3
169761	1	410527	13	NULL	NULL	0	NULL	influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of a 2-day fast was compared with that of a modified fast ( 1.5 g beef protein hydrolysate per kg body wt ) on nitrogen metabolism and insulin secretion in three normal young men .
	manualset3
169762	2	410527	13	NULL	NULL	0	NULL	2-day 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of a 2-day fast was compared with that of a modified fast ( 1.5 g beef protein hydrolysate per kg body wt ) on nitrogen metabolism and insulin secretion in three normal young men .
	manualset3
169763	3	410527	13	NULL	NULL	0	NULL	1.5 g	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of a 2-day fast was compared with that of a modified fast ( 1.5 g beef protein hydrolysate per kg body wt ) on nitrogen metabolism and insulin secretion in three normal young men .
	manualset3
169764	4	410527	13	NULL	NULL	0	NULL	beef protein hydrolysate per kg body wt	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of a 2-day fast was compared with that of a modified fast ( 1.5 g beef protein hydrolysate per kg body wt ) on nitrogen metabolism and insulin secretion in three normal young men .
	manualset3
169765	5	410527	13	NULL	NULL	0	NULL	nitrogen metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of a 2-day fast was compared with that of a modified fast ( 1.5 g beef protein hydrolysate per kg body wt ) on nitrogen metabolism and insulin secretion in three normal young men .
	manualset3
169766	6	410527	13	NULL	NULL	0	NULL	insulin secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of a 2-day fast was compared with that of a modified fast ( 1.5 g beef protein hydrolysate per kg body wt ) on nitrogen metabolism and insulin secretion in three normal young men .
	manualset3
169767	7	410527	13	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of a 2-day fast was compared with that of a modified fast ( 1.5 g beef protein hydrolysate per kg body wt ) on nitrogen metabolism and insulin secretion in three normal young men .
	manualset3
169768	8	410527	13	NULL	NULL	0	NULL	young men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of a 2-day fast was compared with that of a modified fast ( 1.5 g beef protein hydrolysate per kg body wt ) on nitrogen metabolism and insulin secretion in three normal young men .
	manualset3
169769	1	410528	13	NULL	NULL	0	NULL	influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of acyl-PAF and vinyl-PAF on PAF platelet interaction , Ca2 + mobilization , and platelet adenylate cyclase activity is considered .
	manualset3
169770	2	410528	13	NULL	NULL	0	NULL	acyl-PAF 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of acyl-PAF and vinyl-PAF on PAF platelet interaction , Ca2 + mobilization , and platelet adenylate cyclase activity is considered .
	manualset3
169771	3	410528	13	NULL	NULL	0	NULL	vinyl-PAF	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of acyl-PAF and vinyl-PAF on PAF platelet interaction , Ca2 + mobilization , and platelet adenylate cyclase activity is considered .
	manualset3
169772	4	410528	13	NULL	NULL	0	NULL	PAF platelet interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of acyl-PAF and vinyl-PAF on PAF platelet interaction , Ca2 + mobilization , and platelet adenylate cyclase activity is considered .
	manualset3
169773	5	410528	13	NULL	NULL	0	NULL	Ca2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of acyl-PAF and vinyl-PAF on PAF platelet interaction , Ca2 + mobilization , and platelet adenylate cyclase activity is considered .
	manualset3
169774	6	410528	13	NULL	NULL	0	NULL	mobilization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of acyl-PAF and vinyl-PAF on PAF platelet interaction , Ca2 + mobilization , and platelet adenylate cyclase activity is considered .
	manualset3
169775	7	410528	13	NULL	NULL	0	NULL	platelet adenylate cyclase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of acyl-PAF and vinyl-PAF on PAF platelet interaction , Ca2 + mobilization , and platelet adenylate cyclase activity is considered .
	manualset3
169776	1	410529	13	NULL	NULL	0	NULL	influence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of adrenalectomy ( ADX ) on the odor detection performance of male Long-Evans rats was assessed using high-precision olfactometry and a go/no-go operant signal detection task .
	manualset3
169777	2	410529	13	NULL	NULL	0	NULL	adrenalectomy ( ADX )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of adrenalectomy ( ADX ) on the odor detection performance of male Long-Evans rats was assessed using high-precision olfactometry and a go/no-go operant signal detection task .
	manualset3
169778	3	410529	13	NULL	NULL	0	NULL	odor detection performance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of adrenalectomy ( ADX ) on the odor detection performance of male Long-Evans rats was assessed using high-precision olfactometry and a go/no-go operant signal detection task .
	manualset3
169779	4	410529	13	NULL	NULL	0	NULL	male Long-Evans rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of adrenalectomy ( ADX ) on the odor detection performance of male Long-Evans rats was assessed using high-precision olfactometry and a go/no-go operant signal detection task .
	manualset3
169780	5	410529	13	NULL	NULL	0	NULL	high-precision olfactometry 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of adrenalectomy ( ADX ) on the odor detection performance of male Long-Evans rats was assessed using high-precision olfactometry and a go/no-go operant signal detection task .
	manualset3
169781	6	410529	13	NULL	NULL	0	NULL	 go/no-go operant signal detection task	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of adrenalectomy ( ADX ) on the odor detection performance of male Long-Evans rats was assessed using high-precision olfactometry and a go/no-go operant signal detection task .
	manualset3
169782	1	410530	13	NULL	NULL	0	NULL	influence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of anionic surfactant : sodium dodecyl sulfate ( SDS ) and cationic surfactants : cetyltrimethylammonium bromides ( C16TAB ) and cetylpyridinium chloride ( CPC ) on the electronic spectrum of Solophenyl red 3BL azo dye ( C.I. Direct 80 ) in aqueous solution was studied by means of UV-vis spectroscopy .
	manualset3
169783	2	410530	13	NULL	NULL	0	NULL	anionic surfactant	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of anionic surfactant : sodium dodecyl sulfate ( SDS ) and cationic surfactants : cetyltrimethylammonium bromides ( C16TAB ) and cetylpyridinium chloride ( CPC ) on the electronic spectrum of Solophenyl red 3BL azo dye ( C.I. Direct 80 ) in aqueous solution was studied by means of UV-vis spectroscopy .
	manualset3
169784	3	410530	13	NULL	NULL	0	NULL	sodium dodecyl sulfate ( SDS ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of anionic surfactant : sodium dodecyl sulfate ( SDS ) and cationic surfactants : cetyltrimethylammonium bromides ( C16TAB ) and cetylpyridinium chloride ( CPC ) on the electronic spectrum of Solophenyl red 3BL azo dye ( C.I. Direct 80 ) in aqueous solution was studied by means of UV-vis spectroscopy .
	manualset3
169785	4	410530	13	NULL	NULL	0	NULL	cationic surfactants 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of anionic surfactant : sodium dodecyl sulfate ( SDS ) and cationic surfactants : cetyltrimethylammonium bromides ( C16TAB ) and cetylpyridinium chloride ( CPC ) on the electronic spectrum of Solophenyl red 3BL azo dye ( C.I. Direct 80 ) in aqueous solution was studied by means of UV-vis spectroscopy .
	manualset3
169786	5	410530	13	NULL	NULL	0	NULL	cetyltrimethylammonium bromides ( C16TAB )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of anionic surfactant : sodium dodecyl sulfate ( SDS ) and cationic surfactants : cetyltrimethylammonium bromides ( C16TAB ) and cetylpyridinium chloride ( CPC ) on the electronic spectrum of Solophenyl red 3BL azo dye ( C.I. Direct 80 ) in aqueous solution was studied by means of UV-vis spectroscopy .
	manualset3
169787	6	410530	13	NULL	NULL	0	NULL	cetylpyridinium chloride ( CPC )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of anionic surfactant : sodium dodecyl sulfate ( SDS ) and cationic surfactants : cetyltrimethylammonium bromides ( C16TAB ) and cetylpyridinium chloride ( CPC ) on the electronic spectrum of Solophenyl red 3BL azo dye ( C.I. Direct 80 ) in aqueous solution was studied by means of UV-vis spectroscopy .
	manualset3
169788	7	410530	13	NULL	NULL	0	NULL	electronic spectrum	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of anionic surfactant : sodium dodecyl sulfate ( SDS ) and cationic surfactants : cetyltrimethylammonium bromides ( C16TAB ) and cetylpyridinium chloride ( CPC ) on the electronic spectrum of Solophenyl red 3BL azo dye ( C.I. Direct 80 ) in aqueous solution was studied by means of UV-vis spectroscopy .
	manualset3
169789	8	410530	13	NULL	NULL	0	NULL	 Solophenyl red 3BL azo dye ( C.I. Direct 80 ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of anionic surfactant : sodium dodecyl sulfate ( SDS ) and cationic surfactants : cetyltrimethylammonium bromides ( C16TAB ) and cetylpyridinium chloride ( CPC ) on the electronic spectrum of Solophenyl red 3BL azo dye ( C.I. Direct 80 ) in aqueous solution was studied by means of UV-vis spectroscopy .
	manualset3
169790	9	410530	13	NULL	NULL	0	NULL	aqueous solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of anionic surfactant : sodium dodecyl sulfate ( SDS ) and cationic surfactants : cetyltrimethylammonium bromides ( C16TAB ) and cetylpyridinium chloride ( CPC ) on the electronic spectrum of Solophenyl red 3BL azo dye ( C.I. Direct 80 ) in aqueous solution was studied by means of UV-vis spectroscopy .
	manualset3
169791	10	410530	13	NULL	NULL	0	NULL	means 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of anionic surfactant : sodium dodecyl sulfate ( SDS ) and cationic surfactants : cetyltrimethylammonium bromides ( C16TAB ) and cetylpyridinium chloride ( CPC ) on the electronic spectrum of Solophenyl red 3BL azo dye ( C.I. Direct 80 ) in aqueous solution was studied by means of UV-vis spectroscopy .
	manualset3
169792	11	410530	13	NULL	NULL	0	NULL	UV-vis spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of anionic surfactant : sodium dodecyl sulfate ( SDS ) and cationic surfactants : cetyltrimethylammonium bromides ( C16TAB ) and cetylpyridinium chloride ( CPC ) on the electronic spectrum of Solophenyl red 3BL azo dye ( C.I. Direct 80 ) in aqueous solution was studied by means of UV-vis spectroscopy .
	manualset3
170916	1	410531	13	NULL	NULL	0	NULL	influence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of blocking Abs , carbohydrates , full-length glycosylated HIV-1 gp120 envelope protein , and cytochalasin D on the uptake of strains and on the immune responses was determined in vitro .
	manualset3
170917	2	410531	13	NULL	NULL	0	NULL	Abs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of blocking Abs , carbohydrates , full-length glycosylated HIV-1 gp120 envelope protein , and cytochalasin D on the uptake of strains and on the immune responses was determined in vitro .
	manualset3
170918	3	410531	13	NULL	NULL	0	NULL	carbohydrates 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of blocking Abs , carbohydrates , full-length glycosylated HIV-1 gp120 envelope protein , and cytochalasin D on the uptake of strains and on the immune responses was determined in vitro .
	manualset3
170919	4	410531	13	NULL	NULL	0	NULL	full-length glycosylated HIV-1 gp120 envelope protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of blocking Abs , carbohydrates , full-length glycosylated HIV-1 gp120 envelope protein , and cytochalasin D on the uptake of strains and on the immune responses was determined in vitro .
	manualset3
170920	5	410531	13	NULL	NULL	0	NULL	cytochalasin D	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of blocking Abs , carbohydrates , full-length glycosylated HIV-1 gp120 envelope protein , and cytochalasin D on the uptake of strains and on the immune responses was determined in vitro .
	manualset3
170921	6	410531	13	NULL	NULL	0	NULL	uptake 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of blocking Abs , carbohydrates , full-length glycosylated HIV-1 gp120 envelope protein , and cytochalasin D on the uptake of strains and on the immune responses was determined in vitro .
	manualset3
170922	7	410531	13	NULL	NULL	0	NULL	strains 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of blocking Abs , carbohydrates , full-length glycosylated HIV-1 gp120 envelope protein , and cytochalasin D on the uptake of strains and on the immune responses was determined in vitro .
	manualset3
170923	8	410531	13	NULL	NULL	0	NULL	 immune responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of blocking Abs , carbohydrates , full-length glycosylated HIV-1 gp120 envelope protein , and cytochalasin D on the uptake of strains and on the immune responses was determined in vitro .
	manualset3
170924	1	410532	13	NULL	NULL	0	NULL	influence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of combination chemotherapy on antigen expression in ovarian cancer .
	manualset3
170925	2	410532	13	NULL	NULL	0	NULL	combination chemotherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of combination chemotherapy on antigen expression in ovarian cancer .
	manualset3
170926	3	410532	13	NULL	NULL	NULL	NULL	antigen expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The influence of combination chemotherapy on antigen expression in ovarian cancer .
	manualset3
170927	4	410532	13	NULL	NULL	0	NULL	ovarian cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of combination chemotherapy on antigen expression in ovarian cancer .
	manualset3
170928	1	410533	13	NULL	NULL	0	NULL	total 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 118 children between 6 months and 10 years of age with acute urinary tract infection were treated in a random ; double-blind manner with 12 mg/kg/day of trimethoprim-sulfamethoxazole ( 61 patients ) or 50 mg/kg/day of sulfamethoxazole ( 57 patients ) for ten days .
	manualset3
170929	2	410533	13	NULL	NULL	0	NULL	118 children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 118 children between 6 months and 10 years of age with acute urinary tract infection were treated in a random ; double-blind manner with 12 mg/kg/day of trimethoprim-sulfamethoxazole ( 61 patients ) or 50 mg/kg/day of sulfamethoxazole ( 57 patients ) for ten days .
	manualset3
170930	3	410533	13	NULL	NULL	0	NULL	6 months 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 118 children between 6 months and 10 years of age with acute urinary tract infection were treated in a random ; double-blind manner with 12 mg/kg/day of trimethoprim-sulfamethoxazole ( 61 patients ) or 50 mg/kg/day of sulfamethoxazole ( 57 patients ) for ten days .
	manualset3
170931	4	410533	13	NULL	NULL	0	NULL	10 years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 118 children between 6 months and 10 years of age with acute urinary tract infection were treated in a random ; double-blind manner with 12 mg/kg/day of trimethoprim-sulfamethoxazole ( 61 patients ) or 50 mg/kg/day of sulfamethoxazole ( 57 patients ) for ten days .
	manualset3
170932	5	410533	13	NULL	NULL	0	NULL	age 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 118 children between 6 months and 10 years of age with acute urinary tract infection were treated in a random ; double-blind manner with 12 mg/kg/day of trimethoprim-sulfamethoxazole ( 61 patients ) or 50 mg/kg/day of sulfamethoxazole ( 57 patients ) for ten days .
	manualset3
170934	6	410533	13	NULL	NULL	0	NULL	acute urinary tract infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 118 children between 6 months and 10 years of age with acute urinary tract infection were treated in a random ; double-blind manner with 12 mg/kg/day of trimethoprim-sulfamethoxazole ( 61 patients ) or 50 mg/kg/day of sulfamethoxazole ( 57 patients ) for ten days .
	manualset3
170936	8	410533	13	NULL	NULL	0	NULL	double-blind manner	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 118 children between 6 months and 10 years of age with acute urinary tract infection were treated in a random ; double-blind manner with 12 mg/kg/day of trimethoprim-sulfamethoxazole ( 61 patients ) or 50 mg/kg/day of sulfamethoxazole ( 57 patients ) for ten days .
	manualset3
170937	9	410533	13	NULL	NULL	0	NULL	12 mg/kg/day	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 118 children between 6 months and 10 years of age with acute urinary tract infection were treated in a random ; double-blind manner with 12 mg/kg/day of trimethoprim-sulfamethoxazole ( 61 patients ) or 50 mg/kg/day of sulfamethoxazole ( 57 patients ) for ten days .
	manualset3
170938	10	410533	13	NULL	NULL	0	NULL	trimethoprim-sulfamethoxazole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 118 children between 6 months and 10 years of age with acute urinary tract infection were treated in a random ; double-blind manner with 12 mg/kg/day of trimethoprim-sulfamethoxazole ( 61 patients ) or 50 mg/kg/day of sulfamethoxazole ( 57 patients ) for ten days .
	manualset3
170940	11	410533	13	NULL	NULL	0	NULL	61 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 118 children between 6 months and 10 years of age with acute urinary tract infection were treated in a random ; double-blind manner with 12 mg/kg/day of trimethoprim-sulfamethoxazole ( 61 patients ) or 50 mg/kg/day of sulfamethoxazole ( 57 patients ) for ten days .
	manualset3
170941	12	410533	13	NULL	NULL	0	NULL	50 mg/kg/day	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 118 children between 6 months and 10 years of age with acute urinary tract infection were treated in a random ; double-blind manner with 12 mg/kg/day of trimethoprim-sulfamethoxazole ( 61 patients ) or 50 mg/kg/day of sulfamethoxazole ( 57 patients ) for ten days .
	manualset3
170942	13	410533	13	NULL	NULL	0	NULL	sulfamethoxazole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 118 children between 6 months and 10 years of age with acute urinary tract infection were treated in a random ; double-blind manner with 12 mg/kg/day of trimethoprim-sulfamethoxazole ( 61 patients ) or 50 mg/kg/day of sulfamethoxazole ( 57 patients ) for ten days .
	manualset3
170943	14	410533	13	NULL	NULL	0	NULL	57 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 118 children between 6 months and 10 years of age with acute urinary tract infection were treated in a random ; double-blind manner with 12 mg/kg/day of trimethoprim-sulfamethoxazole ( 61 patients ) or 50 mg/kg/day of sulfamethoxazole ( 57 patients ) for ten days .
	manualset3
170944	15	410533	13	NULL	NULL	0	NULL	ten days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 118 children between 6 months and 10 years of age with acute urinary tract infection were treated in a random ; double-blind manner with 12 mg/kg/day of trimethoprim-sulfamethoxazole ( 61 patients ) or 50 mg/kg/day of sulfamethoxazole ( 57 patients ) for ten days .
	manualset3
170945	1	410534	13	NULL	NULL	0	NULL	influence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of damping on the dynamic response of a cantilever must be significant .
	manualset3
170946	2	410534	13	NULL	NULL	0	NULL	response 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of damping on the dynamic response of a cantilever must be significant .
	manualset3
170947	3	410534	13	NULL	NULL	0	NULL	cantilever 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of damping on the dynamic response of a cantilever must be significant .
	manualset3
170948	1	410535	13	NULL	NULL	0	NULL	influence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of gender on the glucose response to exercise remains contradictory .
	manualset3
170949	2	410535	13	NULL	NULL	0	NULL	gender 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of gender on the glucose response to exercise remains contradictory .
	manualset3
170950	3	410535	13	NULL	NULL	0	NULL	glucose response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of gender on the glucose response to exercise remains contradictory .
	manualset3
170951	1	410536	13	NULL	NULL	0	NULL	influence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of induction therapy for kidney transplantation after a non-renal transplant .
	manualset3
170952	2	410536	13	NULL	NULL	0	NULL	induction therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of induction therapy for kidney transplantation after a non-renal transplant .
	manualset3
170953	3	410536	13	NULL	NULL	0	NULL	kidney transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of induction therapy for kidney transplantation after a non-renal transplant .
	manualset3
170954	4	410536	13	NULL	NULL	0	NULL	non-renal transplant	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of induction therapy for kidney transplantation after a non-renal transplant .
	manualset3
170955	1	410537	13	NULL	NULL	0	NULL	influence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of inflammation and coat type on the presence and intensity of estrogen receptor alpha staining was evaluated .
	manualset3
170956	2	410537	13	NULL	NULL	0	NULL	inflammation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of inflammation and coat type on the presence and intensity of estrogen receptor alpha staining was evaluated .
	manualset3
170957	3	410537	13	NULL	NULL	0	NULL	coat type 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of inflammation and coat type on the presence and intensity of estrogen receptor alpha staining was evaluated .
	manualset3
170958	4	410537	13	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of inflammation and coat type on the presence and intensity of estrogen receptor alpha staining was evaluated .
	manualset3
170959	5	410537	13	NULL	NULL	0	NULL	intensity 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of inflammation and coat type on the presence and intensity of estrogen receptor alpha staining was evaluated .
	manualset3
170960	6	410537	13	NULL	NULL	0	NULL	estrogen receptor alpha staining 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of inflammation and coat type on the presence and intensity of estrogen receptor alpha staining was evaluated .
	manualset3
170961	1	410538	13	NULL	NULL	0	NULL	influence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of lipid molecular packing on the affinity of human apolipoprotein A-I ( apo A-I ) for HDL3 and LDL surface lipids was evaluated by monitoring the adsorption of 14C-methylated apo A-I to monolayers of these lipids spread at various initial surface pressures ( pi i ) .
	manualset3
170963	2	410538	13	NULL	NULL	0	NULL	lipid molecular packing	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of lipid molecular packing on the affinity of human apolipoprotein A-I ( apo A-I ) for HDL3 and LDL surface lipids was evaluated by monitoring the adsorption of 14C-methylated apo A-I to monolayers of these lipids spread at various initial surface pressures ( pi i ) .
	manualset3
170964	3	410538	13	NULL	NULL	0	NULL	affinity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of lipid molecular packing on the affinity of human apolipoprotein A-I ( apo A-I ) for HDL3 and LDL surface lipids was evaluated by monitoring the adsorption of 14C-methylated apo A-I to monolayers of these lipids spread at various initial surface pressures ( pi i ) .
	manualset3
170965	4	410538	13	NULL	NULL	0	NULL	human apolipoprotein A-I ( apo A-I )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of lipid molecular packing on the affinity of human apolipoprotein A-I ( apo A-I ) for HDL3 and LDL surface lipids was evaluated by monitoring the adsorption of 14C-methylated apo A-I to monolayers of these lipids spread at various initial surface pressures ( pi i ) .
	manualset3
170966	5	410538	13	NULL	NULL	0	NULL	HDL3 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of lipid molecular packing on the affinity of human apolipoprotein A-I ( apo A-I ) for HDL3 and LDL surface lipids was evaluated by monitoring the adsorption of 14C-methylated apo A-I to monolayers of these lipids spread at various initial surface pressures ( pi i ) .
	manualset3
170967	6	410538	13	NULL	NULL	0	NULL	LDL surface lipids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of lipid molecular packing on the affinity of human apolipoprotein A-I ( apo A-I ) for HDL3 and LDL surface lipids was evaluated by monitoring the adsorption of 14C-methylated apo A-I to monolayers of these lipids spread at various initial surface pressures ( pi i ) .
	manualset3
170968	7	410538	13	NULL	NULL	0	NULL	adsorption 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of lipid molecular packing on the affinity of human apolipoprotein A-I ( apo A-I ) for HDL3 and LDL surface lipids was evaluated by monitoring the adsorption of 14C-methylated apo A-I to monolayers of these lipids spread at various initial surface pressures ( pi i ) .
	manualset3
170969	8	410538	13	NULL	NULL	0	NULL	14C-methylated apo A-I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of lipid molecular packing on the affinity of human apolipoprotein A-I ( apo A-I ) for HDL3 and LDL surface lipids was evaluated by monitoring the adsorption of 14C-methylated apo A-I to monolayers of these lipids spread at various initial surface pressures ( pi i ) .
	manualset3
170970	9	410538	13	NULL	NULL	0	NULL	monolayers 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of lipid molecular packing on the affinity of human apolipoprotein A-I ( apo A-I ) for HDL3 and LDL surface lipids was evaluated by monitoring the adsorption of 14C-methylated apo A-I to monolayers of these lipids spread at various initial surface pressures ( pi i ) .
	manualset3
170971	10	410538	13	NULL	NULL	0	NULL	lipids 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of lipid molecular packing on the affinity of human apolipoprotein A-I ( apo A-I ) for HDL3 and LDL surface lipids was evaluated by monitoring the adsorption of 14C-methylated apo A-I to monolayers of these lipids spread at various initial surface pressures ( pi i ) .
	manualset3
170972	11	410538	13	NULL	NULL	0	NULL	initial surface pressures ( pi i ) 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of lipid molecular packing on the affinity of human apolipoprotein A-I ( apo A-I ) for HDL3 and LDL surface lipids was evaluated by monitoring the adsorption of 14C-methylated apo A-I to monolayers of these lipids spread at various initial surface pressures ( pi i ) .
	manualset3
170973	1	410539	13	NULL	NULL	0	NULL	influence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of povidone-iodine treatment on thyroid hormones in severe burns .
	manualset3
170974	2	410539	13	NULL	NULL	0	NULL	povidone-iodine treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of povidone-iodine treatment on thyroid hormones in severe burns .
	manualset3
170975	3	410539	13	NULL	NULL	0	NULL	thyroid hormones	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of povidone-iodine treatment on thyroid hormones in severe burns .
	manualset3
170976	4	410539	13	NULL	NULL	0	NULL	burns 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of povidone-iodine treatment on thyroid hormones in severe burns .
	manualset3
170977	1	410540	13	NULL	NULL	0	NULL	influence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of religious factors on drinking behavior among young indigenous sami and non-sami peers in northern norway .
	manualset3
170979	2	410540	13	NULL	NULL	0	NULL	religious factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of religious factors on drinking behavior among young indigenous sami and non-sami peers in northern norway .
	manualset3
170980	3	410540	13	NULL	NULL	0	NULL	drinking behavior	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of religious factors on drinking behavior among young indigenous sami and non-sami peers in northern norway .
	manualset3
170981	4	410540	13	NULL	NULL	0	NULL	young indigenous sami peers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of religious factors on drinking behavior among young indigenous sami and non-sami peers in northern norway .
	manualset3
170982	5	410540	13	NULL	NULL	0	NULL	non-sami peers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of religious factors on drinking behavior among young indigenous sami and non-sami peers in northern norway .
	manualset3
170983	6	410540	13	NULL	NULL	0	NULL	northern norway	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of religious factors on drinking behavior among young indigenous sami and non-sami peers in northern norway .
	manualset3
170984	1	410541	13	NULL	NULL	0	NULL	influence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of route of administration , schedule of administration and dose on the pharmacokinetics of ifosfamide and its metabolites are discussed .
	manualset3
170985	2	410541	13	NULL	NULL	0	NULL	route 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of route of administration , schedule of administration and dose on the pharmacokinetics of ifosfamide and its metabolites are discussed .
	manualset3
170986	3	410541	13	NULL	NULL	0	NULL	administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of route of administration , schedule of administration and dose on the pharmacokinetics of ifosfamide and its metabolites are discussed .
	manualset3
170987	4	410541	13	NULL	NULL	0	NULL	schedule of administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of route of administration , schedule of administration and dose on the pharmacokinetics of ifosfamide and its metabolites are discussed .
	manualset3
170988	5	410541	13	NULL	NULL	0	NULL	dose 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of route of administration , schedule of administration and dose on the pharmacokinetics of ifosfamide and its metabolites are discussed .
	manualset3
170989	6	410541	13	NULL	NULL	0	NULL	pharmacokinetics 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of route of administration , schedule of administration and dose on the pharmacokinetics of ifosfamide and its metabolites are discussed .
	manualset3
170990	7	410541	13	NULL	NULL	0	NULL	ifosfamide 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of route of administration , schedule of administration and dose on the pharmacokinetics of ifosfamide and its metabolites are discussed .
	manualset3
170991	8	410541	13	NULL	NULL	0	NULL	metabolites 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of route of administration , schedule of administration and dose on the pharmacokinetics of ifosfamide and its metabolites are discussed .
	manualset3
170992	1	410542	13	NULL	NULL	0	NULL	influence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of route of administration on wound fluid concentration of prophylactic antibiotics .
	manualset3
170993	2	410542	13	NULL	NULL	0	NULL	route of administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of route of administration on wound fluid concentration of prophylactic antibiotics .
	manualset3
170994	3	410542	13	NULL	NULL	0	NULL	wound fluid concentration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of route of administration on wound fluid concentration of prophylactic antibiotics .
	manualset3
170995	4	410542	13	NULL	NULL	0	NULL	prophylactic antibiotics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of route of administration on wound fluid concentration of prophylactic antibiotics .
	manualset3
170996	1	410543	13	NULL	NULL	0	NULL	influence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of sodium bromide in man : a study in human volunteers with special emphasis on the endocrine and the central nervous system .
	manualset3
170998	2	410543	13	NULL	NULL	0	NULL	sodium bromide 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of sodium bromide in man : a study in human volunteers with special emphasis on the endocrine and the central nervous system .
	manualset3
170999	3	410543	13	NULL	NULL	0	NULL	man 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of sodium bromide in man : a study in human volunteers with special emphasis on the endocrine and the central nervous system .
	manualset3
171000	4	410543	13	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of sodium bromide in man : a study in human volunteers with special emphasis on the endocrine and the central nervous system .
	manualset3
171001	5	410543	13	NULL	NULL	0	NULL	human volunteers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of sodium bromide in man : a study in human volunteers with special emphasis on the endocrine and the central nervous system .
	manualset3
171002	6	410543	13	NULL	NULL	0	NULL	emphasis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of sodium bromide in man : a study in human volunteers with special emphasis on the endocrine and the central nervous system .
	manualset3
171003	7	410543	13	NULL	NULL	0	NULL	endocrine system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of sodium bromide in man : a study in human volunteers with special emphasis on the endocrine and the central nervous system .
	manualset3
171004	8	410543	13	NULL	NULL	0	NULL	central nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of sodium bromide in man : a study in human volunteers with special emphasis on the endocrine and the central nervous system .
	manualset3
171005	1	410544	13	NULL	NULL	0	NULL	influence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of specific pseudomonad populations and volatile organic compounds ( VOC ) on primordium formation of A. bisporus was studied in microcosm cultures .
	manualset3
171006	2	410544	13	NULL	NULL	0	NULL	pseudomonad populations 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of specific pseudomonad populations and volatile organic compounds ( VOC ) on primordium formation of A. bisporus was studied in microcosm cultures .
	manualset3
171007	3	410544	13	NULL	NULL	0	NULL	volatile organic compounds ( VOC ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of specific pseudomonad populations and volatile organic compounds ( VOC ) on primordium formation of A. bisporus was studied in microcosm cultures .
	manualset3
171008	4	410544	13	NULL	NULL	0	NULL	primordium formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of specific pseudomonad populations and volatile organic compounds ( VOC ) on primordium formation of A. bisporus was studied in microcosm cultures .
	manualset3
171009	5	410544	13	NULL	NULL	0	NULL	A. bisporus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of specific pseudomonad populations and volatile organic compounds ( VOC ) on primordium formation of A. bisporus was studied in microcosm cultures .
	manualset3
171010	6	410544	13	NULL	NULL	0	NULL	microcosm cultures	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of specific pseudomonad populations and volatile organic compounds ( VOC ) on primordium formation of A. bisporus was studied in microcosm cultures .
	manualset3
171011	1	410545	13	NULL	NULL	0	NULL	influence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of subintimal angioplasty on level of amputation and limb salvage rates in lower limb critical ischemia : a 15-year experience .
	manualset3
171013	2	410545	13	NULL	NULL	0	NULL	subintimal angioplasty	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of subintimal angioplasty on level of amputation and limb salvage rates in lower limb critical ischemia : a 15-year experience .
	manualset3
171016	3	410545	13	NULL	NULL	0	NULL	level 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of subintimal angioplasty on level of amputation and limb salvage rates in lower limb critical ischemia : a 15-year experience .
	manualset3
171017	4	410545	13	NULL	NULL	0	NULL	amputation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of subintimal angioplasty on level of amputation and limb salvage rates in lower limb critical ischemia : a 15-year experience .
	manualset3
171018	5	410545	13	NULL	NULL	0	NULL	limb salvage rates 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of subintimal angioplasty on level of amputation and limb salvage rates in lower limb critical ischemia : a 15-year experience .
	manualset3
171019	6	410545	13	NULL	NULL	0	NULL	lower limb critical ischemia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of subintimal angioplasty on level of amputation and limb salvage rates in lower limb critical ischemia : a 15-year experience .
	manualset3
171020	7	410545	13	NULL	NULL	0	NULL	15-year	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of subintimal angioplasty on level of amputation and limb salvage rates in lower limb critical ischemia : a 15-year experience .
	manualset3
171021	8	410545	13	NULL	NULL	0	NULL	experience 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of subintimal angioplasty on level of amputation and limb salvage rates in lower limb critical ischemia : a 15-year experience .
	manualset3
171022	1	410546	13	NULL	NULL	0	NULL	influence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of the autonomic nervous system on sinus node automatism was assessed in 61 patients with suspect sinus node dysfunction .
	manualset3
171023	2	410546	13	NULL	NULL	0	NULL	autonomic nervous system 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of the autonomic nervous system on sinus node automatism was assessed in 61 patients with suspect sinus node dysfunction .
	manualset3
171024	3	410546	13	NULL	NULL	0	NULL	sinus node automatism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of the autonomic nervous system on sinus node automatism was assessed in 61 patients with suspect sinus node dysfunction .
	manualset3
171025	4	410546	13	NULL	NULL	0	NULL	61 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of the autonomic nervous system on sinus node automatism was assessed in 61 patients with suspect sinus node dysfunction .
	manualset3
171026	5	410546	13	NULL	NULL	0	NULL	sinus node dysfunction 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of the autonomic nervous system on sinus node automatism was assessed in 61 patients with suspect sinus node dysfunction .
	manualset3
171027	1	410547	13	NULL	NULL	0	NULL	influence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of the particle releasing position is mainly shown near the nasal valve region for micron particle deposition , while for submicron particles deposition , both the nasal valve and turbinate region are influenced .
	manualset3
171032	2	410547	13	NULL	NULL	0	NULL	particle 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of the particle releasing position is mainly shown near the nasal valve region for micron particle deposition , while for submicron particles deposition , both the nasal valve and turbinate region are influenced .
	manualset3
171033	3	410547	13	NULL	NULL	0	NULL	position 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of the particle releasing position is mainly shown near the nasal valve region for micron particle deposition , while for submicron particles deposition , both the nasal valve and turbinate region are influenced .
	manualset3
171034	4	410547	13	NULL	NULL	0	NULL	nasal valve region	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of the particle releasing position is mainly shown near the nasal valve region for micron particle deposition , while for submicron particles deposition , both the nasal valve and turbinate region are influenced .
	manualset3
171035	5	410547	13	NULL	NULL	0	NULL	micron particle deposition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of the particle releasing position is mainly shown near the nasal valve region for micron particle deposition , while for submicron particles deposition , both the nasal valve and turbinate region are influenced .
	manualset3
171036	6	410547	13	NULL	NULL	0	NULL	submicron particles deposition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of the particle releasing position is mainly shown near the nasal valve region for micron particle deposition , while for submicron particles deposition , both the nasal valve and turbinate region are influenced .
	manualset3
171037	7	410547	13	NULL	NULL	0	NULL	nasal valve	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of the particle releasing position is mainly shown near the nasal valve region for micron particle deposition , while for submicron particles deposition , both the nasal valve and turbinate region are influenced .
	manualset3
171038	8	410547	13	NULL	NULL	0	NULL	turbinate region 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of the particle releasing position is mainly shown near the nasal valve region for micron particle deposition , while for submicron particles deposition , both the nasal valve and turbinate region are influenced .
	manualset3
171039	1	410548	13	NULL	NULL	0	NULL	influence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of tobacco smoke on indoor atmosphere .
	manualset3
171040	2	410548	13	NULL	NULL	0	NULL	tobacco smoke	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of tobacco smoke on indoor atmosphere .
	manualset3
171041	3	410548	13	NULL	NULL	0	NULL	indoor atmosphere 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of tobacco smoke on indoor atmosphere .
	manualset3
171042	1	410549	13	NULL	NULL	0	NULL	influence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of type of photosensitizer , drug and light dose , and time interval between photosensitizer and illumination on the extent of photodynamic therapy ( PDT ) - induced bladder damage and recovery was investigated using a mouse model .
	manualset3
171043	2	410549	13	NULL	NULL	0	NULL	type of photosensitizer	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of type of photosensitizer , drug and light dose , and time interval between photosensitizer and illumination on the extent of photodynamic therapy ( PDT ) - induced bladder damage and recovery was investigated using a mouse model .
	manualset3
171044	3	410549	13	NULL	NULL	0	NULL	drug 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of type of photosensitizer , drug and light dose , and time interval between photosensitizer and illumination on the extent of photodynamic therapy ( PDT ) - induced bladder damage and recovery was investigated using a mouse model .
	manualset3
171045	4	410549	13	NULL	NULL	0	NULL	light dose	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of type of photosensitizer , drug and light dose , and time interval between photosensitizer and illumination on the extent of photodynamic therapy ( PDT ) - induced bladder damage and recovery was investigated using a mouse model .
	manualset3
171046	5	410549	13	NULL	NULL	0	NULL	time interval	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of type of photosensitizer , drug and light dose , and time interval between photosensitizer and illumination on the extent of photodynamic therapy ( PDT ) - induced bladder damage and recovery was investigated using a mouse model .
	manualset3
171047	6	410549	13	NULL	NULL	0	NULL	photosensitizer	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of type of photosensitizer , drug and light dose , and time interval between photosensitizer and illumination on the extent of photodynamic therapy ( PDT ) - induced bladder damage and recovery was investigated using a mouse model .
	manualset3
171048	7	410549	13	NULL	NULL	0	NULL	illumination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of type of photosensitizer , drug and light dose , and time interval between photosensitizer and illumination on the extent of photodynamic therapy ( PDT ) - induced bladder damage and recovery was investigated using a mouse model .
	manualset3
171049	8	410549	13	NULL	NULL	0	NULL	photodynamic therapy ( PDT )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of type of photosensitizer , drug and light dose , and time interval between photosensitizer and illumination on the extent of photodynamic therapy ( PDT ) - induced bladder damage and recovery was investigated using a mouse model .
	manualset3
171050	9	410549	13	NULL	NULL	0	NULL	bladder damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of type of photosensitizer , drug and light dose , and time interval between photosensitizer and illumination on the extent of photodynamic therapy ( PDT ) - induced bladder damage and recovery was investigated using a mouse model .
	manualset3
171051	10	410549	13	NULL	NULL	0	NULL	recovery 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of type of photosensitizer , drug and light dose , and time interval between photosensitizer and illumination on the extent of photodynamic therapy ( PDT ) - induced bladder damage and recovery was investigated using a mouse model .
	manualset3
171052	11	410549	13	NULL	NULL	0	NULL	mouse model 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of type of photosensitizer , drug and light dose , and time interval between photosensitizer and illumination on the extent of photodynamic therapy ( PDT ) - induced bladder damage and recovery was investigated using a mouse model .
	manualset3
171103	1	410550	13	NULL	NULL	0	NULL	influences	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influences of the interpositus nucleus on pyramidal tract neurons were investigated by stimulating , in unanesthetized cats , interpositus nucleus foci which activated single muscles in limbs , while recording unitary discharges of pyramidal tract neurons located in foci ( area 4 gamma ) from which contraction was obtained in the same muscles as those excited from interpositus nucleus ( agonist pyramidal tract neurons ) , in their antagonist ( antagonist pyramidal tract neurons ) , or in heteronymous muscles ( heteronymous pyramidal tract neurons ) .
	manualset3
171104	2	410550	13	NULL	NULL	0	NULL	interpositus nucleus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The influences of the interpositus nucleus on pyramidal tract neurons were investigated by stimulating , in unanesthetized cats , interpositus nucleus foci which activated single muscles in limbs , while recording unitary discharges of pyramidal tract neurons located in foci ( area 4 gamma ) from which contraction was obtained in the same muscles as those excited from interpositus nucleus ( agonist pyramidal tract neurons ) , in their antagonist ( antagonist pyramidal tract neurons ) , or in heteronymous muscles ( heteronymous pyramidal tract neurons ) .
	manualset3
171105	3	410550	13	NULL	NULL	0	NULL	pyramidal tract neurons	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The influences of the interpositus nucleus on pyramidal tract neurons were investigated by stimulating , in unanesthetized cats , interpositus nucleus foci which activated single muscles in limbs , while recording unitary discharges of pyramidal tract neurons located in foci ( area 4 gamma ) from which contraction was obtained in the same muscles as those excited from interpositus nucleus ( agonist pyramidal tract neurons ) , in their antagonist ( antagonist pyramidal tract neurons ) , or in heteronymous muscles ( heteronymous pyramidal tract neurons ) .
	manualset3
171106	4	410550	13	NULL	NULL	0	NULL	cats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The influences of the interpositus nucleus on pyramidal tract neurons were investigated by stimulating , in unanesthetized cats , interpositus nucleus foci which activated single muscles in limbs , while recording unitary discharges of pyramidal tract neurons located in foci ( area 4 gamma ) from which contraction was obtained in the same muscles as those excited from interpositus nucleus ( agonist pyramidal tract neurons ) , in their antagonist ( antagonist pyramidal tract neurons ) , or in heteronymous muscles ( heteronymous pyramidal tract neurons ) .
	manualset3
171107	5	410550	13	NULL	NULL	0	NULL	interpositus nucleus foci	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The influences of the interpositus nucleus on pyramidal tract neurons were investigated by stimulating , in unanesthetized cats , interpositus nucleus foci which activated single muscles in limbs , while recording unitary discharges of pyramidal tract neurons located in foci ( area 4 gamma ) from which contraction was obtained in the same muscles as those excited from interpositus nucleus ( agonist pyramidal tract neurons ) , in their antagonist ( antagonist pyramidal tract neurons ) , or in heteronymous muscles ( heteronymous pyramidal tract neurons ) .
	manualset3
171108	6	410550	13	NULL	NULL	0	NULL	muscles 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The influences of the interpositus nucleus on pyramidal tract neurons were investigated by stimulating , in unanesthetized cats , interpositus nucleus foci which activated single muscles in limbs , while recording unitary discharges of pyramidal tract neurons located in foci ( area 4 gamma ) from which contraction was obtained in the same muscles as those excited from interpositus nucleus ( agonist pyramidal tract neurons ) , in their antagonist ( antagonist pyramidal tract neurons ) , or in heteronymous muscles ( heteronymous pyramidal tract neurons ) .
	manualset3
171109	7	410550	13	NULL	NULL	0	NULL	limbs 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The influences of the interpositus nucleus on pyramidal tract neurons were investigated by stimulating , in unanesthetized cats , interpositus nucleus foci which activated single muscles in limbs , while recording unitary discharges of pyramidal tract neurons located in foci ( area 4 gamma ) from which contraction was obtained in the same muscles as those excited from interpositus nucleus ( agonist pyramidal tract neurons ) , in their antagonist ( antagonist pyramidal tract neurons ) , or in heteronymous muscles ( heteronymous pyramidal tract neurons ) .
	manualset3
171110	8	410550	13	NULL	NULL	0	NULL	unitary discharges	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influences of the interpositus nucleus on pyramidal tract neurons were investigated by stimulating , in unanesthetized cats , interpositus nucleus foci which activated single muscles in limbs , while recording unitary discharges of pyramidal tract neurons located in foci ( area 4 gamma ) from which contraction was obtained in the same muscles as those excited from interpositus nucleus ( agonist pyramidal tract neurons ) , in their antagonist ( antagonist pyramidal tract neurons ) , or in heteronymous muscles ( heteronymous pyramidal tract neurons ) .
	manualset3
171111	9	410550	13	NULL	NULL	0	NULL	pyramidal tract neurons 	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The influences of the interpositus nucleus on pyramidal tract neurons were investigated by stimulating , in unanesthetized cats , interpositus nucleus foci which activated single muscles in limbs , while recording unitary discharges of pyramidal tract neurons located in foci ( area 4 gamma ) from which contraction was obtained in the same muscles as those excited from interpositus nucleus ( agonist pyramidal tract neurons ) , in their antagonist ( antagonist pyramidal tract neurons ) , or in heteronymous muscles ( heteronymous pyramidal tract neurons ) .
	manualset3
171112	10	410550	13	NULL	NULL	0	NULL	foci 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The influences of the interpositus nucleus on pyramidal tract neurons were investigated by stimulating , in unanesthetized cats , interpositus nucleus foci which activated single muscles in limbs , while recording unitary discharges of pyramidal tract neurons located in foci ( area 4 gamma ) from which contraction was obtained in the same muscles as those excited from interpositus nucleus ( agonist pyramidal tract neurons ) , in their antagonist ( antagonist pyramidal tract neurons ) , or in heteronymous muscles ( heteronymous pyramidal tract neurons ) .
	manualset3
171113	11	410550	13	NULL	NULL	0	NULL	area 4 gamma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The influences of the interpositus nucleus on pyramidal tract neurons were investigated by stimulating , in unanesthetized cats , interpositus nucleus foci which activated single muscles in limbs , while recording unitary discharges of pyramidal tract neurons located in foci ( area 4 gamma ) from which contraction was obtained in the same muscles as those excited from interpositus nucleus ( agonist pyramidal tract neurons ) , in their antagonist ( antagonist pyramidal tract neurons ) , or in heteronymous muscles ( heteronymous pyramidal tract neurons ) .
	manualset3
171114	12	410550	13	NULL	NULL	0	NULL	contraction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The influences of the interpositus nucleus on pyramidal tract neurons were investigated by stimulating , in unanesthetized cats , interpositus nucleus foci which activated single muscles in limbs , while recording unitary discharges of pyramidal tract neurons located in foci ( area 4 gamma ) from which contraction was obtained in the same muscles as those excited from interpositus nucleus ( agonist pyramidal tract neurons ) , in their antagonist ( antagonist pyramidal tract neurons ) , or in heteronymous muscles ( heteronymous pyramidal tract neurons ) .
	manualset3
171115	13	410550	13	NULL	NULL	0	NULL	muscles 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The influences of the interpositus nucleus on pyramidal tract neurons were investigated by stimulating , in unanesthetized cats , interpositus nucleus foci which activated single muscles in limbs , while recording unitary discharges of pyramidal tract neurons located in foci ( area 4 gamma ) from which contraction was obtained in the same muscles as those excited from interpositus nucleus ( agonist pyramidal tract neurons ) , in their antagonist ( antagonist pyramidal tract neurons ) , or in heteronymous muscles ( heteronymous pyramidal tract neurons ) .
	manualset3
171116	14	410550	13	NULL	NULL	0	NULL	interpositus nucleus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The influences of the interpositus nucleus on pyramidal tract neurons were investigated by stimulating , in unanesthetized cats , interpositus nucleus foci which activated single muscles in limbs , while recording unitary discharges of pyramidal tract neurons located in foci ( area 4 gamma ) from which contraction was obtained in the same muscles as those excited from interpositus nucleus ( agonist pyramidal tract neurons ) , in their antagonist ( antagonist pyramidal tract neurons ) , or in heteronymous muscles ( heteronymous pyramidal tract neurons ) .
	manualset3
171118	15	410550	13	NULL	NULL	0	NULL	agonist pyramidal tract neurons 	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The influences of the interpositus nucleus on pyramidal tract neurons were investigated by stimulating , in unanesthetized cats , interpositus nucleus foci which activated single muscles in limbs , while recording unitary discharges of pyramidal tract neurons located in foci ( area 4 gamma ) from which contraction was obtained in the same muscles as those excited from interpositus nucleus ( agonist pyramidal tract neurons ) , in their antagonist ( antagonist pyramidal tract neurons ) , or in heteronymous muscles ( heteronymous pyramidal tract neurons ) .
	manualset3
171119	16	410550	13	NULL	NULL	0	NULL	antagonist 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The influences of the interpositus nucleus on pyramidal tract neurons were investigated by stimulating , in unanesthetized cats , interpositus nucleus foci which activated single muscles in limbs , while recording unitary discharges of pyramidal tract neurons located in foci ( area 4 gamma ) from which contraction was obtained in the same muscles as those excited from interpositus nucleus ( agonist pyramidal tract neurons ) , in their antagonist ( antagonist pyramidal tract neurons ) , or in heteronymous muscles ( heteronymous pyramidal tract neurons ) .
	manualset3
171120	17	410550	13	NULL	NULL	0	NULL	antagonist pyramidal tract neurons	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The influences of the interpositus nucleus on pyramidal tract neurons were investigated by stimulating , in unanesthetized cats , interpositus nucleus foci which activated single muscles in limbs , while recording unitary discharges of pyramidal tract neurons located in foci ( area 4 gamma ) from which contraction was obtained in the same muscles as those excited from interpositus nucleus ( agonist pyramidal tract neurons ) , in their antagonist ( antagonist pyramidal tract neurons ) , or in heteronymous muscles ( heteronymous pyramidal tract neurons ) .
	manualset3
171121	18	410550	13	NULL	NULL	0	NULL	heteronymous muscles 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The influences of the interpositus nucleus on pyramidal tract neurons were investigated by stimulating , in unanesthetized cats , interpositus nucleus foci which activated single muscles in limbs , while recording unitary discharges of pyramidal tract neurons located in foci ( area 4 gamma ) from which contraction was obtained in the same muscles as those excited from interpositus nucleus ( agonist pyramidal tract neurons ) , in their antagonist ( antagonist pyramidal tract neurons ) , or in heteronymous muscles ( heteronymous pyramidal tract neurons ) .
	manualset3
171122	19	410550	13	NULL	NULL	0	NULL	heteronymous pyramidal tract neurons	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The influences of the interpositus nucleus on pyramidal tract neurons were investigated by stimulating , in unanesthetized cats , interpositus nucleus foci which activated single muscles in limbs , while recording unitary discharges of pyramidal tract neurons located in foci ( area 4 gamma ) from which contraction was obtained in the same muscles as those excited from interpositus nucleus ( agonist pyramidal tract neurons ) , in their antagonist ( antagonist pyramidal tract neurons ) , or in heteronymous muscles ( heteronymous pyramidal tract neurons ) .
	manualset3
171123	1	410551	13	NULL	NULL	0	NULL	informants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The informants had different opinions on whether letter or telephone was the best method for first contact .
	manualset3
171124	2	410551	13	NULL	NULL	0	NULL	opinions 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The informants had different opinions on whether letter or telephone was the best method for first contact .
	manualset3
171125	3	410551	13	NULL	NULL	0	NULL	letter 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The informants had different opinions on whether letter or telephone was the best method for first contact .
	manualset3
171126	4	410551	13	NULL	NULL	0	NULL	telephone 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The informants had different opinions on whether letter or telephone was the best method for first contact .
	manualset3
171128	5	410551	13	NULL	NULL	0	NULL	method 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The informants had different opinions on whether letter or telephone was the best method for first contact .
	manualset3
171129	6	410551	13	NULL	NULL	0	NULL	contact 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The informants had different opinions on whether letter or telephone was the best method for first contact .
	manualset3
171130	1	410552	13	NULL	NULL	0	NULL	information 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The information from the registration can lead to primary or secondary prevention ( prevention of the disease or of its complications , respectively ) .
	manualset3
171131	2	410552	13	NULL	NULL	0	NULL	registration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The information from the registration can lead to primary or secondary prevention ( prevention of the disease or of its complications , respectively ) .
	manualset3
171132	3	410552	13	NULL	NULL	0	NULL	primary prevention 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The information from the registration can lead to primary or secondary prevention ( prevention of the disease or of its complications , respectively ) .
	manualset3
171133	4	410552	13	NULL	NULL	0	NULL	secondary prevention 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The information from the registration can lead to primary or secondary prevention ( prevention of the disease or of its complications , respectively ) .
	manualset3
171134	5	410552	13	NULL	NULL	0	NULL	prevention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The information from the registration can lead to primary or secondary prevention ( prevention of the disease or of its complications , respectively ) .
	manualset3
171135	6	410552	13	NULL	NULL	0	NULL	disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The information from the registration can lead to primary or secondary prevention ( prevention of the disease or of its complications , respectively ) .
	manualset3
171136	7	410552	13	NULL	NULL	0	NULL	complications 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The information from the registration can lead to primary or secondary prevention ( prevention of the disease or of its complications , respectively ) .
	manualset3
171137	1	410553	13	NULL	NULL	0	NULL	information 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The information is used to control the amount of cladding removed from a D fiber to within approximately 0.05 microm for use in the production of passive optical fiber components .
	manualset3
171138	2	410553	13	NULL	NULL	0	NULL	amount 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The information is used to control the amount of cladding removed from a D fiber to within approximately 0.05 microm for use in the production of passive optical fiber components .
	manualset3
171139	3	410553	13	NULL	NULL	0	NULL	cladding 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The information is used to control the amount of cladding removed from a D fiber to within approximately 0.05 microm for use in the production of passive optical fiber components .
	manualset3
171140	4	410553	13	NULL	NULL	0	NULL	D fiber	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The information is used to control the amount of cladding removed from a D fiber to within approximately 0.05 microm for use in the production of passive optical fiber components .
	manualset3
171141	5	410553	13	NULL	NULL	0	NULL	approximately 0.05 microm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The information is used to control the amount of cladding removed from a D fiber to within approximately 0.05 microm for use in the production of passive optical fiber components .
	manualset3
171142	6	410553	13	NULL	NULL	0	NULL	use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The information is used to control the amount of cladding removed from a D fiber to within approximately 0.05 microm for use in the production of passive optical fiber components .
	manualset3
171143	7	410553	13	NULL	NULL	0	NULL	production 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The information is used to control the amount of cladding removed from a D fiber to within approximately 0.05 microm for use in the production of passive optical fiber components .
	manualset3
171144	8	410553	13	NULL	NULL	NULL	NULL	passive optical fiber components 	Thing												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The information is used to control the amount of cladding removed from a D fiber to within approximately 0.05 microm for use in the production of passive optical fiber components .
	manualset3
171146	1	410554	13	NULL	NULL	0	NULL	information 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The information obtained also demonstrated that hope interacts with nearly all domains in the Sunrise Model .
	manualset3
171147	2	410554	13	NULL	NULL	0	NULL	hope 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The information obtained also demonstrated that hope interacts with nearly all domains in the Sunrise Model .
	manualset3
171148	3	410554	13	NULL	NULL	0	NULL	domains 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The information obtained also demonstrated that hope interacts with nearly all domains in the Sunrise Model .
	manualset3
171150	4	410554	13	NULL	NULL	0	NULL	Sunrise Model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The information obtained also demonstrated that hope interacts with nearly all domains in the Sunrise Model .
	manualset3
171151	1	410555	13	NULL	NULL	0	NULL	information technology age	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The information technology age is dawning for medical education .
	manualset3
171152	2	410555	13	NULL	NULL	0	NULL	medical education	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The information technology age is dawning for medical education .
	manualset3
171169	1	410556	13	NULL	NULL	0	NULL	information 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The information was analyzed using the SPSS 13.0 program .
	manualset3
171171	2	410556	13	NULL	NULL	0	NULL	SPSS 13.0 program 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The information was analyzed using the SPSS 13.0 program .
	manualset3
171172	1	410557	13	NULL	NULL	0	NULL	infrastructure 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The infrastructure for primary and community care must , however , be put in place before acute facilities are shut .
	manualset3
171173	2	410557	13	NULL	NULL	0	NULL	primary care 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The infrastructure for primary and community care must , however , be put in place before acute facilities are shut .
	manualset3
171174	3	410557	13	NULL	NULL	0	NULL	community care 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The infrastructure for primary and community care must , however , be put in place before acute facilities are shut .
	manualset3
171175	4	410557	13	NULL	NULL	0	NULL	acute facilities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The infrastructure for primary and community care must , however , be put in place before acute facilities are shut .
	manualset3
171176	5	410557	13	NULL	NULL	NULL	NULL	place 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The infrastructure for primary and community care must , however , be put in place before acute facilities are shut .
	manualset3
171177	1	410558	13	NULL	NULL	0	NULL	inhibition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition is dependent on the dose of gamone added ; the structural conformation and the relative concentration of the inhibitor ; and the time of addition of the inhibitor .
	manualset3
171178	2	410558	13	NULL	NULL	0	NULL	dose 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition is dependent on the dose of gamone added ; the structural conformation and the relative concentration of the inhibitor ; and the time of addition of the inhibitor .
	manualset3
171179	3	410558	13	NULL	NULL	0	NULL	gamone 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition is dependent on the dose of gamone added ; the structural conformation and the relative concentration of the inhibitor ; and the time of addition of the inhibitor .
	manualset3
171180	4	410558	13	NULL	NULL	0	NULL	conformation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition is dependent on the dose of gamone added ; the structural conformation and the relative concentration of the inhibitor ; and the time of addition of the inhibitor .
	manualset3
171181	5	410558	13	NULL	NULL	0	NULL	concentration 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition is dependent on the dose of gamone added ; the structural conformation and the relative concentration of the inhibitor ; and the time of addition of the inhibitor .
	manualset3
171183	6	410558	13	NULL	NULL	0	NULL	inhibitor 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition is dependent on the dose of gamone added ; the structural conformation and the relative concentration of the inhibitor ; and the time of addition of the inhibitor .
	manualset3
171184	7	410558	13	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition is dependent on the dose of gamone added ; the structural conformation and the relative concentration of the inhibitor ; and the time of addition of the inhibitor .
	manualset3
171185	8	410558	13	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition is dependent on the dose of gamone added ; the structural conformation and the relative concentration of the inhibitor ; and the time of addition of the inhibitor .
	manualset3
171187	9	410558	13	NULL	NULL	0	NULL	inhibitor 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition is dependent on the dose of gamone added ; the structural conformation and the relative concentration of the inhibitor ; and the time of addition of the inhibitor .
	manualset3
171188	1	410559	13	NULL	NULL	0	NULL	inhibition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition of K ( + ) ( ATP ) channels with glibenclamide attenuated the ursolic acid-induced increase in ANP secretion-but not atrial dynamics-in a concentration-dependent manner .
	manualset3
171189	2	410559	13	NULL	NULL	0	NULL	K ( + ) ( ATP ) channels	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition of K ( + ) ( ATP ) channels with glibenclamide attenuated the ursolic acid-induced increase in ANP secretion-but not atrial dynamics-in a concentration-dependent manner .
	manualset3
171190	3	410559	13	NULL	NULL	0	NULL	glibenclamide 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition of K ( + ) ( ATP ) channels with glibenclamide attenuated the ursolic acid-induced increase in ANP secretion-but not atrial dynamics-in a concentration-dependent manner .
	manualset3
171191	4	410559	13	NULL	NULL	NULL	NULL	ursolic acid-induced increase 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The inhibition of K ( + ) ( ATP ) channels with glibenclamide attenuated the ursolic acid-induced increase in ANP secretion-but not atrial dynamics-in a concentration-dependent manner .
	manualset3
171192	5	410559	13	NULL	NULL	0	NULL	ANP 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition of K ( + ) ( ATP ) channels with glibenclamide attenuated the ursolic acid-induced increase in ANP secretion-but not atrial dynamics-in a concentration-dependent manner .
	manualset3
171194	6	410559	13	NULL	NULL	0	NULL	concentration-dependent manner 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition of K ( + ) ( ATP ) channels with glibenclamide attenuated the ursolic acid-induced increase in ANP secretion-but not atrial dynamics-in a concentration-dependent manner .
	manualset3
171195	1	410560	13	NULL	NULL	0	NULL	inhibition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition of cancer cell proliferation highly correlated with the levels of polyphenols , flavonoids and their antioxidant activities .
	manualset3
171196	2	410560	13	NULL	NULL	0	NULL	cancer cell proliferation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition of cancer cell proliferation highly correlated with the levels of polyphenols , flavonoids and their antioxidant activities .
	manualset3
171197	3	410560	13	NULL	NULL	0	NULL	levels 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition of cancer cell proliferation highly correlated with the levels of polyphenols , flavonoids and their antioxidant activities .
	manualset3
171198	4	410560	13	NULL	NULL	0	NULL	polyphenols 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition of cancer cell proliferation highly correlated with the levels of polyphenols , flavonoids and their antioxidant activities .
	manualset3
171199	5	410560	13	NULL	NULL	0	NULL	flavonoids 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition of cancer cell proliferation highly correlated with the levels of polyphenols , flavonoids and their antioxidant activities .
	manualset3
171200	6	410560	13	NULL	NULL	0	NULL	antioxidant activities 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition of cancer cell proliferation highly correlated with the levels of polyphenols , flavonoids and their antioxidant activities .
	manualset3
171201	1	410561	13	NULL	NULL	0	NULL	Clinical aspects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical aspects and differential diagnosis of acute dysentery and other diarrheal diseases ) .
	manualset3
171202	2	410561	13	NULL	NULL	NULL	NULL	differential diagnosis 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Clinical aspects and differential diagnosis of acute dysentery and other diarrheal diseases ) .
	manualset3
171203	3	410561	13	NULL	NULL	0	NULL	acute dysentery	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical aspects and differential diagnosis of acute dysentery and other diarrheal diseases ) .
	manualset3
171205	4	410561	13	NULL	NULL	0	NULL	diarrheal diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical aspects and differential diagnosis of acute dysentery and other diarrheal diseases ) .
	manualset3
171206	1	410562	13	NULL	NULL	0	NULL	total 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 150 DNA samples from 150 Okinawan patients with head and neck squamous cell carcinoma ( HNSCC ) were screened for HPV sequences by PCR using three consensus primer sets , and HPV types were determined by direct sequencing .
	manualset3
171207	2	410562	13	NULL	NULL	0	NULL	150 DNA samples 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 150 DNA samples from 150 Okinawan patients with head and neck squamous cell carcinoma ( HNSCC ) were screened for HPV sequences by PCR using three consensus primer sets , and HPV types were determined by direct sequencing .
	manualset3
171208	3	410562	13	NULL	NULL	0	NULL	150 Okinawan patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 150 DNA samples from 150 Okinawan patients with head and neck squamous cell carcinoma ( HNSCC ) were screened for HPV sequences by PCR using three consensus primer sets , and HPV types were determined by direct sequencing .
	manualset3
171209	4	410562	13	NULL	NULL	0	NULL	head and neck squamous cell carcinoma ( HNSCC )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 150 DNA samples from 150 Okinawan patients with head and neck squamous cell carcinoma ( HNSCC ) were screened for HPV sequences by PCR using three consensus primer sets , and HPV types were determined by direct sequencing .
	manualset3
171210	5	410562	13	NULL	NULL	0	NULL	HPV sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 150 DNA samples from 150 Okinawan patients with head and neck squamous cell carcinoma ( HNSCC ) were screened for HPV sequences by PCR using three consensus primer sets , and HPV types were determined by direct sequencing .
	manualset3
171211	6	410562	13	NULL	NULL	0	NULL	PCR 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 150 DNA samples from 150 Okinawan patients with head and neck squamous cell carcinoma ( HNSCC ) were screened for HPV sequences by PCR using three consensus primer sets , and HPV types were determined by direct sequencing .
	manualset3
171212	7	410562	13	NULL	NULL	0	NULL	three consensus primer sets	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 150 DNA samples from 150 Okinawan patients with head and neck squamous cell carcinoma ( HNSCC ) were screened for HPV sequences by PCR using three consensus primer sets , and HPV types were determined by direct sequencing .
	manualset3
171213	8	410562	13	NULL	NULL	0	NULL	HPV types	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 150 DNA samples from 150 Okinawan patients with head and neck squamous cell carcinoma ( HNSCC ) were screened for HPV sequences by PCR using three consensus primer sets , and HPV types were determined by direct sequencing .
	manualset3
171214	9	410562	13	NULL	NULL	0	NULL	direct sequencing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 150 DNA samples from 150 Okinawan patients with head and neck squamous cell carcinoma ( HNSCC ) were screened for HPV sequences by PCR using three consensus primer sets , and HPV types were determined by direct sequencing .
	manualset3
171291	1	410563	13	NULL	NULL	0	NULL	inhibition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition of iNOS expression by the GLP-1 / cyclic AMP/PKA pathway might possibly be of therapeutic potential in NO-mediated beta-cell dysfunction and destruction .
	manualset3
171292	2	410563	13	NULL	NULL	0	NULL	iNOS expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition of iNOS expression by the GLP-1 / cyclic AMP/PKA pathway might possibly be of therapeutic potential in NO-mediated beta-cell dysfunction and destruction .
	manualset3
171293	3	410563	13	NULL	NULL	0	NULL	GLP-1 / cyclic AMP/PKA pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition of iNOS expression by the GLP-1 / cyclic AMP/PKA pathway might possibly be of therapeutic potential in NO-mediated beta-cell dysfunction and destruction .
	manualset3
171294	4	410563	13	NULL	NULL	0	NULL	therapeutic potential	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition of iNOS expression by the GLP-1 / cyclic AMP/PKA pathway might possibly be of therapeutic potential in NO-mediated beta-cell dysfunction and destruction .
	manualset3
171295	5	410563	13	NULL	NULL	0	NULL	NO-mediated beta-cell dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition of iNOS expression by the GLP-1 / cyclic AMP/PKA pathway might possibly be of therapeutic potential in NO-mediated beta-cell dysfunction and destruction .
	manualset3
171296	6	410563	13	NULL	NULL	0	NULL	destruction 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition of iNOS expression by the GLP-1 / cyclic AMP/PKA pathway might possibly be of therapeutic potential in NO-mediated beta-cell dysfunction and destruction .
	manualset3
171297	1	410564	13	NULL	NULL	0	NULL	inhibition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition of infection is shown to occur at an early stage , and can be reversed if the cells express gene II in addition to gene V protein .
	manualset3
171298	2	410564	13	NULL	NULL	0	NULL	infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition of infection is shown to occur at an early stage , and can be reversed if the cells express gene II in addition to gene V protein .
	manualset3
171299	3	410564	13	NULL	NULL	0	NULL	early stage	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition of infection is shown to occur at an early stage , and can be reversed if the cells express gene II in addition to gene V protein .
	manualset3
171300	4	410564	13	NULL	NULL	0	NULL	cells 	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition of infection is shown to occur at an early stage , and can be reversed if the cells express gene II in addition to gene V protein .
	manualset3
171301	5	410564	13	NULL	NULL	0	NULL	gene II 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition of infection is shown to occur at an early stage , and can be reversed if the cells express gene II in addition to gene V protein .
	manualset3
171302	6	410564	13	NULL	NULL	0	NULL	gene V protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition of infection is shown to occur at an early stage , and can be reversed if the cells express gene II in addition to gene V protein .
	manualset3
171303	1	410565	13	NULL	NULL	0	NULL	inhibition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition of integrin alpha2 expression in HUVEC showed dose dependence but did not alter the level of CD31 .
	manualset3
171304	2	410565	13	NULL	NULL	0	NULL	integrin alpha2 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition of integrin alpha2 expression in HUVEC showed dose dependence but did not alter the level of CD31 .
	manualset3
171305	3	410565	13	NULL	NULL	0	NULL	HUVEC 	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition of integrin alpha2 expression in HUVEC showed dose dependence but did not alter the level of CD31 .
	manualset3
171306	4	410565	13	NULL	NULL	0	NULL	dose 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition of integrin alpha2 expression in HUVEC showed dose dependence but did not alter the level of CD31 .
	manualset3
171307	5	410565	13	NULL	NULL	0	NULL	dependence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition of integrin alpha2 expression in HUVEC showed dose dependence but did not alter the level of CD31 .
	manualset3
171308	6	410565	13	NULL	NULL	0	NULL	level 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition of integrin alpha2 expression in HUVEC showed dose dependence but did not alter the level of CD31 .
	manualset3
171309	7	410565	13	NULL	NULL	0	NULL	CD31 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibition of integrin alpha2 expression in HUVEC showed dose dependence but did not alter the level of CD31 .
	manualset3
171310	1	410566	13	NULL	NULL	0	NULL	inhibitors 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitors bis-indolylmaleimide I and PD98059 blocked ERK1/2 phosphorylation and completely eliminated angiotensin stimulation of the CCT-catalyzed reaction and PC synthesis .
	manualset3
171311	2	410566	13	NULL	NULL	0	NULL	bis-indolylmaleimide I	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitors bis-indolylmaleimide I and PD98059 blocked ERK1/2 phosphorylation and completely eliminated angiotensin stimulation of the CCT-catalyzed reaction and PC synthesis .
	manualset3
171313	3	410566	13	NULL	NULL	0	NULL	PD98059 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitors bis-indolylmaleimide I and PD98059 blocked ERK1/2 phosphorylation and completely eliminated angiotensin stimulation of the CCT-catalyzed reaction and PC synthesis .
	manualset3
171314	4	410566	13	NULL	NULL	0	NULL	ERK1/2 phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitors bis-indolylmaleimide I and PD98059 blocked ERK1/2 phosphorylation and completely eliminated angiotensin stimulation of the CCT-catalyzed reaction and PC synthesis .
	manualset3
171315	5	410566	13	NULL	NULL	0	NULL	angiotensin stimulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitors bis-indolylmaleimide I and PD98059 blocked ERK1/2 phosphorylation and completely eliminated angiotensin stimulation of the CCT-catalyzed reaction and PC synthesis .
	manualset3
171316	6	410566	13	NULL	NULL	0	NULL	CCT-catalyzed reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitors bis-indolylmaleimide I and PD98059 blocked ERK1/2 phosphorylation and completely eliminated angiotensin stimulation of the CCT-catalyzed reaction and PC synthesis .
	manualset3
171317	7	410566	13	NULL	NULL	0	NULL	PC synthesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitors bis-indolylmaleimide I and PD98059 blocked ERK1/2 phosphorylation and completely eliminated angiotensin stimulation of the CCT-catalyzed reaction and PC synthesis .
	manualset3
171318	1	410567	13	NULL	NULL	0	NULL	inhibitory activities 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory activities of NO production by these compounds and their chemical derivatives in lipopolysaccharide and TNF - activated macrophage-like cell line J774 .1 were tested .
	manualset3
171320	2	410567	13	NULL	NULL	0	NULL	NO production 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory activities of NO production by these compounds and their chemical derivatives in lipopolysaccharide and TNF - activated macrophage-like cell line J774 .1 were tested .
	manualset3
171321	3	410567	13	NULL	NULL	0	NULL	compounds 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory activities of NO production by these compounds and their chemical derivatives in lipopolysaccharide and TNF - activated macrophage-like cell line J774 .1 were tested .
	manualset3
171322	4	410567	13	NULL	NULL	0	NULL	chemical derivatives 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory activities of NO production by these compounds and their chemical derivatives in lipopolysaccharide and TNF - activated macrophage-like cell line J774 .1 were tested .
	manualset3
171323	5	410567	13	NULL	NULL	0	NULL	lipopolysaccharide 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory activities of NO production by these compounds and their chemical derivatives in lipopolysaccharide and TNF - activated macrophage-like cell line J774 .1 were tested .
	manualset3
171324	6	410567	13	NULL	NULL	0	NULL	macrophage-like cell line J774 .1	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory activities of NO production by these compounds and their chemical derivatives in lipopolysaccharide and TNF - activated macrophage-like cell line J774 .1 were tested .
	manualset3
171325	1	410568	13	NULL	NULL	0	NULL	inhibitory effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory effects of three calcium blockers , diltiazem ( d-form ) , verapamil , and nifedipine , on ADP - and collagen-induced platelet aggregation of human and rabbit platelets were compared .
	manualset3
171326	2	410568	13	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory effects of three calcium blockers , diltiazem ( d-form ) , verapamil , and nifedipine , on ADP - and collagen-induced platelet aggregation of human and rabbit platelets were compared .
	manualset3
171327	3	410568	13	NULL	NULL	0	NULL	calcium blockers	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory effects of three calcium blockers , diltiazem ( d-form ) , verapamil , and nifedipine , on ADP - and collagen-induced platelet aggregation of human and rabbit platelets were compared .
	manualset3
171328	4	410568	13	NULL	NULL	0	NULL	diltiazem ( d-form )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory effects of three calcium blockers , diltiazem ( d-form ) , verapamil , and nifedipine , on ADP - and collagen-induced platelet aggregation of human and rabbit platelets were compared .
	manualset3
171329	5	410568	13	NULL	NULL	0	NULL	verapamil 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory effects of three calcium blockers , diltiazem ( d-form ) , verapamil , and nifedipine , on ADP - and collagen-induced platelet aggregation of human and rabbit platelets were compared .
	manualset3
171330	6	410568	13	NULL	NULL	0	NULL	nifedipine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory effects of three calcium blockers , diltiazem ( d-form ) , verapamil , and nifedipine , on ADP - and collagen-induced platelet aggregation of human and rabbit platelets were compared .
	manualset3
171331	7	410568	13	NULL	NULL	0	NULL	platelet aggregation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory effects of three calcium blockers , diltiazem ( d-form ) , verapamil , and nifedipine , on ADP - and collagen-induced platelet aggregation of human and rabbit platelets were compared .
	manualset3
171332	8	410568	13	NULL	NULL	0	NULL	human platelets 	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory effects of three calcium blockers , diltiazem ( d-form ) , verapamil , and nifedipine , on ADP - and collagen-induced platelet aggregation of human and rabbit platelets were compared .
	manualset3
171333	9	410568	13	NULL	NULL	0	NULL	rabbit platelets 	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory effects of three calcium blockers , diltiazem ( d-form ) , verapamil , and nifedipine , on ADP - and collagen-induced platelet aggregation of human and rabbit platelets were compared .
	manualset3
171335	1	410569	13	NULL	NULL	0	NULL	inhibitory effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory effects on CDK2 appear to be transcriptional .
	manualset3
171336	2	410569	13	NULL	NULL	0	NULL	CDK2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory effects on CDK2 appear to be transcriptional .
	manualset3
171337	1	410570	13	NULL	NULL	0	NULL	inhibitory potency	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory potency of G-actin on poly ( A ) polymerase was reduced after co-incubation with DNase I or phalloidin and that of tubulin by colchicine .
	manualset3
171338	2	410570	13	NULL	NULL	0	NULL	G-actin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory potency of G-actin on poly ( A ) polymerase was reduced after co-incubation with DNase I or phalloidin and that of tubulin by colchicine .
	manualset3
171339	3	410570	13	NULL	NULL	0	NULL	poly ( A ) polymerase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory potency of G-actin on poly ( A ) polymerase was reduced after co-incubation with DNase I or phalloidin and that of tubulin by colchicine .
	manualset3
171341	4	410570	13	NULL	NULL	0	NULL	co-incubation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory potency of G-actin on poly ( A ) polymerase was reduced after co-incubation with DNase I or phalloidin and that of tubulin by colchicine .
	manualset3
178667	5	410570	13	NULL	NULL	0	NULL	DNase I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory potency of G-actin on poly ( A ) polymerase was reduced after co-incubation with DNase I or phalloidin and that of tubulin by colchicine .
	manualset3
178668	6	410570	13	NULL	NULL	0	NULL	phalloidin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory potency of G-actin on poly ( A ) polymerase was reduced after co-incubation with DNase I or phalloidin and that of tubulin by colchicine .
	manualset3
178669	7	410570	13	NULL	NULL	0	NULL	 tubulin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory potency of G-actin on poly ( A ) polymerase was reduced after co-incubation with DNase I or phalloidin and that of tubulin by colchicine .
	manualset3
178670	8	410570	13	NULL	NULL	0	NULL	colchicine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory potency of G-actin on poly ( A ) polymerase was reduced after co-incubation with DNase I or phalloidin and that of tubulin by colchicine .
	manualset3
171977	1	410571	13	NULL	NULL	0	NULL	inhibitory preparations	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory preparations of CP-S-S-OVA and CP-S-S-CP were shown to be inactive in an ELISA for human IgG directed against the unrelated benzylpenicilloyl antigen .
	manualset3
171978	2	410571	13	NULL	NULL	0	NULL	CP-S-S-OVA	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory preparations of CP-S-S-OVA and CP-S-S-CP were shown to be inactive in an ELISA for human IgG directed against the unrelated benzylpenicilloyl antigen .
	manualset3
171979	3	410571	13	NULL	NULL	0	NULL	CP-S-S-CP	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory preparations of CP-S-S-OVA and CP-S-S-CP were shown to be inactive in an ELISA for human IgG directed against the unrelated benzylpenicilloyl antigen .
	manualset3
171980	4	410571	13	NULL	NULL	0	NULL	 ELISA 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory preparations of CP-S-S-OVA and CP-S-S-CP were shown to be inactive in an ELISA for human IgG directed against the unrelated benzylpenicilloyl antigen .
	manualset3
171981	5	410571	13	NULL	NULL	0	NULL	human IgG	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory preparations of CP-S-S-OVA and CP-S-S-CP were shown to be inactive in an ELISA for human IgG directed against the unrelated benzylpenicilloyl antigen .
	manualset3
171982	6	410571	13	NULL	NULL	0	NULL	benzylpenicilloyl antigen	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory preparations of CP-S-S-OVA and CP-S-S-CP were shown to be inactive in an ELISA for human IgG directed against the unrelated benzylpenicilloyl antigen .
	manualset3
172218	1	410572	13	NULL	NULL	0	NULL	initial strain states	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial and final strain states of the rolled-up oxide layers are studied by X-ray diffraction on an ensemble of tubes .
	manualset3
172219	2	410572	13	NULL	NULL	0	NULL	final strain states	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial and final strain states of the rolled-up oxide layers are studied by X-ray diffraction on an ensemble of tubes .
	manualset3
172220	3	410572	13	NULL	NULL	0	NULL	oxide layers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial and final strain states of the rolled-up oxide layers are studied by X-ray diffraction on an ensemble of tubes .
	manualset3
172221	4	410572	13	NULL	NULL	0	NULL	X-ray diffraction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial and final strain states of the rolled-up oxide layers are studied by X-ray diffraction on an ensemble of tubes .
	manualset3
172222	5	410572	13	NULL	NULL	0	NULL	ensemble	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial and final strain states of the rolled-up oxide layers are studied by X-ray diffraction on an ensemble of tubes .
	manualset3
172223	6	410572	13	NULL	NULL	0	NULL	tubes	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial and final strain states of the rolled-up oxide layers are studied by X-ray diffraction on an ensemble of tubes .
	manualset3
172224	1	410573	13	NULL	NULL	0	NULL	classification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial classification recognized only two categories : primary pulmonary hypertension and secondary pulmonary hypertension , depending on the presence or absence of identified causes or risk factors .
	manualset3
172225	2	410573	13	NULL	NULL	0	NULL	two categories 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial classification recognized only two categories : primary pulmonary hypertension and secondary pulmonary hypertension , depending on the presence or absence of identified causes or risk factors .
	manualset3
172226	3	410573	13	NULL	NULL	0	NULL	primary pulmonary hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial classification recognized only two categories : primary pulmonary hypertension and secondary pulmonary hypertension , depending on the presence or absence of identified causes or risk factors .
	manualset3
172227	4	410573	13	NULL	NULL	0	NULL	secondary pulmonary hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial classification recognized only two categories : primary pulmonary hypertension and secondary pulmonary hypertension , depending on the presence or absence of identified causes or risk factors .
	manualset3
172228	5	410573	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial classification recognized only two categories : primary pulmonary hypertension and secondary pulmonary hypertension , depending on the presence or absence of identified causes or risk factors .
	manualset3
172229	6	410573	13	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial classification recognized only two categories : primary pulmonary hypertension and secondary pulmonary hypertension , depending on the presence or absence of identified causes or risk factors .
	manualset3
172230	7	410573	13	NULL	NULL	0	NULL	causes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial classification recognized only two categories : primary pulmonary hypertension and secondary pulmonary hypertension , depending on the presence or absence of identified causes or risk factors .
	manualset3
172231	8	410573	13	NULL	NULL	0	NULL	risk factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial classification recognized only two categories : primary pulmonary hypertension and secondary pulmonary hypertension , depending on the presence or absence of identified causes or risk factors .
	manualset3
172232	1	410574	13	NULL	NULL	0	NULL	complex	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial complex lacks coordination of the LBA carboxylate ( C-1 ) and is bound by the `` 2 , 3 , 5 '' hydroxyl groups .
	manualset3
172233	2	410574	13	NULL	NULL	0	NULL	coordination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial complex lacks coordination of the LBA carboxylate ( C-1 ) and is bound by the `` 2 , 3 , 5 '' hydroxyl groups .
	manualset3
172234	3	410574	13	NULL	NULL	0	NULL	LBA carboxylate ( C-1 ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial complex lacks coordination of the LBA carboxylate ( C-1 ) and is bound by the `` 2 , 3 , 5 '' hydroxyl groups .
	manualset3
172235	4	410574	13	NULL	NULL	0	NULL	`` 2 , 3 , 5 '' hydroxyl groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial complex lacks coordination of the LBA carboxylate ( C-1 ) and is bound by the `` 2 , 3 , 5 '' hydroxyl groups .
	manualset3
172236	1	410575	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial increase in calcium produced by hydrogen peroxide was not affected by EGTA , but was partially prevented by dithiothreitol .
	manualset3
172237	2	410575	13	NULL	NULL	0	NULL	calcium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial increase in calcium produced by hydrogen peroxide was not affected by EGTA , but was partially prevented by dithiothreitol .
	manualset3
172238	3	410575	13	NULL	NULL	0	NULL	hydrogen peroxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial increase in calcium produced by hydrogen peroxide was not affected by EGTA , but was partially prevented by dithiothreitol .
	manualset3
172239	4	410575	13	NULL	NULL	0	NULL	EGTA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial increase in calcium produced by hydrogen peroxide was not affected by EGTA , but was partially prevented by dithiothreitol .
	manualset3
172240	5	410575	13	NULL	NULL	0	NULL	dithiothreitol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial increase in calcium produced by hydrogen peroxide was not affected by EGTA , but was partially prevented by dithiothreitol .
	manualset3
172241	1	410576	13	NULL	NULL	0	NULL	pneumogram	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial pneumogram was obtained at a mean age of 6.9 weeks , and the repeat pneumogram 2.3 weeks later , when the mean theophylline blood concentration was 11.2 + / - 0.5 micrograms/ml .
	manualset3
172242	2	410576	13	NULL	NULL	0	NULL	mean age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial pneumogram was obtained at a mean age of 6.9 weeks , and the repeat pneumogram 2.3 weeks later , when the mean theophylline blood concentration was 11.2 + / - 0.5 micrograms/ml .
	manualset3
172243	3	410576	13	NULL	NULL	0	NULL	6.9 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial pneumogram was obtained at a mean age of 6.9 weeks , and the repeat pneumogram 2.3 weeks later , when the mean theophylline blood concentration was 11.2 + / - 0.5 micrograms/ml .
	manualset3
172244	4	410576	13	NULL	NULL	0	NULL	repeat pneumogram	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial pneumogram was obtained at a mean age of 6.9 weeks , and the repeat pneumogram 2.3 weeks later , when the mean theophylline blood concentration was 11.2 + / - 0.5 micrograms/ml .
	manualset3
172245	5	410576	13	NULL	NULL	0	NULL	2.3 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial pneumogram was obtained at a mean age of 6.9 weeks , and the repeat pneumogram 2.3 weeks later , when the mean theophylline blood concentration was 11.2 + / - 0.5 micrograms/ml .
	manualset3
172246	6	410576	13	NULL	NULL	0	NULL	theophylline	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial pneumogram was obtained at a mean age of 6.9 weeks , and the repeat pneumogram 2.3 weeks later , when the mean theophylline blood concentration was 11.2 + / - 0.5 micrograms/ml .
	manualset3
172248	7	410576	13	NULL	NULL	0	NULL	blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial pneumogram was obtained at a mean age of 6.9 weeks , and the repeat pneumogram 2.3 weeks later , when the mean theophylline blood concentration was 11.2 + / - 0.5 micrograms/ml .
	manualset3
172249	8	410576	13	NULL	NULL	0	NULL	concentration 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial pneumogram was obtained at a mean age of 6.9 weeks , and the repeat pneumogram 2.3 weeks later , when the mean theophylline blood concentration was 11.2 + / - 0.5 micrograms/ml .
	manualset3
172251	9	410576	13	NULL	NULL	0	NULL	11.2 + / - 0.5 micrograms/ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial pneumogram was obtained at a mean age of 6.9 weeks , and the repeat pneumogram 2.3 weeks later , when the mean theophylline blood concentration was 11.2 + / - 0.5 micrograms/ml .
	manualset3
172260	1	410577	13	NULL	NULL	0	NULL	rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial rate of 2.3 mumol/min per g of cells proceeded for approx .
	manualset3
172261	2	410577	13	NULL	NULL	0	NULL	2.3 mumol/min per g 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial rate of 2.3 mumol/min per g of cells proceeded for approx .
	manualset3
172262	3	410577	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial rate of 2.3 mumol/min per g of cells proceeded for approx .
	manualset3
172263	4	410577	13	NULL	NULL	0	NULL	approx	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial rate of 2.3 mumol/min per g of cells proceeded for approx .
	manualset3
172266	1	410578	13	NULL	NULL	0	NULL	 reference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial reference was the examination at 2 weeks , which was compared to subsequent follow-up .
	manualset3
172267	2	410578	13	NULL	NULL	0	NULL	examination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial reference was the examination at 2 weeks , which was compared to subsequent follow-up .
	manualset3
172268	3	410578	13	NULL	NULL	0	NULL	2 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial reference was the examination at 2 weeks , which was compared to subsequent follow-up .
	manualset3
172269	4	410578	13	NULL	NULL	0	NULL	follow-up	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial reference was the examination at 2 weeks , which was compared to subsequent follow-up .
	manualset3
172329	1	410579	13	NULL	NULL	0	NULL	restraint 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial restraint led to significant increases in ACTH , cortisol , prolactin , and GH concentrations .
	manualset3
172331	2	410579	13	NULL	NULL	0	NULL	increases	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial restraint led to significant increases in ACTH , cortisol , prolactin , and GH concentrations .
	manualset3
172334	3	410579	13	NULL	NULL	0	NULL	ACTH	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial restraint led to significant increases in ACTH , cortisol , prolactin , and GH concentrations .
	manualset3
172335	4	410579	13	NULL	NULL	0	NULL	cortisol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial restraint led to significant increases in ACTH , cortisol , prolactin , and GH concentrations .
	manualset3
172337	5	410579	13	NULL	NULL	0	NULL	prolactin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial restraint led to significant increases in ACTH , cortisol , prolactin , and GH concentrations .
	manualset3
172339	6	410579	13	NULL	NULL	0	NULL	GH	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial restraint led to significant increases in ACTH , cortisol , prolactin , and GH concentrations .
	manualset3
172341	7	410579	13	NULL	NULL	0	NULL	concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial restraint led to significant increases in ACTH , cortisol , prolactin , and GH concentrations .
	manualset3
172345	1	410580	13	NULL	NULL	0	NULL	initial stages 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial stages of delirium are frequently confused with anxiety .
	manualset3
172346	2	410580	13	NULL	NULL	0	NULL	delirium	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial stages of delirium are frequently confused with anxiety .
	manualset3
172347	3	410580	13	NULL	NULL	0	NULL	anxiety 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial stages of delirium are frequently confused with anxiety .
	manualset3
172348	1	410581	13	NULL	NULL	0	NULL	thyroid Tc-99m pertechnetate scan	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial thyroid Tc-99m pertechnetate scan demonstrated decreased uptake in the entire left lobe of the thyroid .
	manualset3
172349	2	410581	13	NULL	NULL	0	NULL	uptake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial thyroid Tc-99m pertechnetate scan demonstrated decreased uptake in the entire left lobe of the thyroid .
	manualset3
172350	3	410581	13	NULL	NULL	0	NULL	left lobe	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial thyroid Tc-99m pertechnetate scan demonstrated decreased uptake in the entire left lobe of the thyroid .
	manualset3
172351	4	410581	13	NULL	NULL	0	NULL	thyroid	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial thyroid Tc-99m pertechnetate scan demonstrated decreased uptake in the entire left lobe of the thyroid .
	manualset3
172352	1	410582	13	NULL	NULL	0	NULL	event	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The initiating event in preeclampsia has been postulated to be reduced uteroplacental perfusion .
	manualset3
172353	2	410582	13	NULL	NULL	0	NULL	preeclampsia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The initiating event in preeclampsia has been postulated to be reduced uteroplacental perfusion .
	manualset3
172354	3	410582	13	NULL	NULL	0	NULL	uteroplacental perfusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The initiating event in preeclampsia has been postulated to be reduced uteroplacental perfusion .
	manualset3
172355	1	410583	13	NULL	NULL	0	NULL	initiative 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The initiative has also allowed researchers to hurdle many of the barricades that have hindered accurate analysis such as the lack of reference standards and comparative data .
	manualset3
172356	2	410583	13	NULL	NULL	0	NULL	researchers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The initiative has also allowed researchers to hurdle many of the barricades that have hindered accurate analysis such as the lack of reference standards and comparative data .
	manualset3
172367	3	410583	13	NULL	NULL	0	NULL	barricades	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The initiative has also allowed researchers to hurdle many of the barricades that have hindered accurate analysis such as the lack of reference standards and comparative data .
	manualset3
172368	4	410583	13	NULL	NULL	0	NULL	analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The initiative has also allowed researchers to hurdle many of the barricades that have hindered accurate analysis such as the lack of reference standards and comparative data .
	manualset3
172369	5	410583	13	NULL	NULL	0	NULL	lack	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The initiative has also allowed researchers to hurdle many of the barricades that have hindered accurate analysis such as the lack of reference standards and comparative data .
	manualset3
172371	6	410583	13	NULL	NULL	0	NULL	reference standards 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The initiative has also allowed researchers to hurdle many of the barricades that have hindered accurate analysis such as the lack of reference standards and comparative data .
	manualset3
172373	7	410583	13	NULL	NULL	0	NULL	comparative data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The initiative has also allowed researchers to hurdle many of the barricades that have hindered accurate analysis such as the lack of reference standards and comparative data .
	manualset3
172374	1	410584	13	NULL	NULL	0	NULL	initiator tRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The initiator tRNA must serve functions distinct from those of other tRNAs , evading binding to elongation factors and instead binding directly to the ribosomal P site with the aid of initiation factors .
	manualset3
172375	2	410584	13	NULL	NULL	0	NULL	functions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The initiator tRNA must serve functions distinct from those of other tRNAs , evading binding to elongation factors and instead binding directly to the ribosomal P site with the aid of initiation factors .
	manualset3
172376	3	410584	13	NULL	NULL	0	NULL	tRNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The initiator tRNA must serve functions distinct from those of other tRNAs , evading binding to elongation factors and instead binding directly to the ribosomal P site with the aid of initiation factors .
	manualset3
172377	4	410584	13	NULL	NULL	0	NULL	elongation factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The initiator tRNA must serve functions distinct from those of other tRNAs , evading binding to elongation factors and instead binding directly to the ribosomal P site with the aid of initiation factors .
	manualset3
172378	5	410584	13	NULL	NULL	0	NULL	ribosomal P site	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The initiator tRNA must serve functions distinct from those of other tRNAs , evading binding to elongation factors and instead binding directly to the ribosomal P site with the aid of initiation factors .
	manualset3
172379	6	410584	13	NULL	NULL	0	NULL	aid	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The initiator tRNA must serve functions distinct from those of other tRNAs , evading binding to elongation factors and instead binding directly to the ribosomal P site with the aid of initiation factors .
	manualset3
172380	7	410584	13	NULL	NULL	0	NULL	initiation factors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The initiator tRNA must serve functions distinct from those of other tRNAs , evading binding to elongation factors and instead binding directly to the ribosomal P site with the aid of initiation factors .
	manualset3
172381	1	410585	13	NULL	NULL	0	NULL	injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The injury and LLLT procedures were then repeated 15 hours later on the same tendon .
	manualset3
172382	2	410585	13	NULL	NULL	0	NULL	LLLT procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The injury and LLLT procedures were then repeated 15 hours later on the same tendon .
	manualset3
172383	3	410585	13	NULL	NULL	0	NULL	15 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The injury and LLLT procedures were then repeated 15 hours later on the same tendon .
	manualset3
172384	4	410585	13	NULL	NULL	0	NULL	tendon	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The injury and LLLT procedures were then repeated 15 hours later on the same tendon .
	manualset3
172385	1	410586	13	NULL	NULL	0	NULL	insight	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The insight that we have gained through our GWAS sets the stage for the rational development of novel effective therapeutic approaches and heralds in an exciting new era with the commencement of translational research in AA based on genetic findings .
	manualset3
172477	2	410586	13	NULL	NULL	0	NULL	GWAS sets	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The insight that we have gained through our GWAS sets the stage for the rational development of novel effective therapeutic approaches and heralds in an exciting new era with the commencement of translational research in AA based on genetic findings .
	manualset3
172478	3	410586	13	NULL	NULL	0	NULL	stage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The insight that we have gained through our GWAS sets the stage for the rational development of novel effective therapeutic approaches and heralds in an exciting new era with the commencement of translational research in AA based on genetic findings .
	manualset3
172479	4	410586	13	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The insight that we have gained through our GWAS sets the stage for the rational development of novel effective therapeutic approaches and heralds in an exciting new era with the commencement of translational research in AA based on genetic findings .
	manualset3
172480	5	410586	13	NULL	NULL	0	NULL	therapeutic approaches 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The insight that we have gained through our GWAS sets the stage for the rational development of novel effective therapeutic approaches and heralds in an exciting new era with the commencement of translational research in AA based on genetic findings .
	manualset3
172481	6	410586	13	NULL	NULL	0	NULL	heralds	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The insight that we have gained through our GWAS sets the stage for the rational development of novel effective therapeutic approaches and heralds in an exciting new era with the commencement of translational research in AA based on genetic findings .
	manualset3
172482	7	410586	13	NULL	NULL	0	NULL	era	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The insight that we have gained through our GWAS sets the stage for the rational development of novel effective therapeutic approaches and heralds in an exciting new era with the commencement of translational research in AA based on genetic findings .
	manualset3
172483	8	410586	13	NULL	NULL	NULL	NULL	commencement	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The insight that we have gained through our GWAS sets the stage for the rational development of novel effective therapeutic approaches and heralds in an exciting new era with the commencement of translational research in AA based on genetic findings .
	manualset3
172484	9	410586	13	NULL	NULL	0	NULL	translational research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The insight that we have gained through our GWAS sets the stage for the rational development of novel effective therapeutic approaches and heralds in an exciting new era with the commencement of translational research in AA based on genetic findings .
	manualset3
172485	10	410586	13	NULL	NULL	0	NULL	alopecia areata	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The insight that we have gained through our GWAS sets the stage for the rational development of novel effective therapeutic approaches and heralds in an exciting new era with the commencement of translational research in AA based on genetic findings .
	manualset3
172486	11	410586	13	NULL	NULL	0	NULL	genetic findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The insight that we have gained through our GWAS sets the stage for the rational development of novel effective therapeutic approaches and heralds in an exciting new era with the commencement of translational research in AA based on genetic findings .
	manualset3
172487	1	410587	13	NULL	NULL	0	NULL	instrument	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The instrument is basically an implementation of the cross-correlation between the excitation source and the induced fluorescence response .
	manualset3
172488	2	410587	13	NULL	NULL	0	NULL	implementation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The instrument is basically an implementation of the cross-correlation between the excitation source and the induced fluorescence response .
	manualset3
172489	3	410587	13	NULL	NULL	0	NULL	cross-correlation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The instrument is basically an implementation of the cross-correlation between the excitation source and the induced fluorescence response .
	manualset3
172490	4	410587	13	NULL	NULL	0	NULL	excitation source	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The instrument is basically an implementation of the cross-correlation between the excitation source and the induced fluorescence response .
	manualset3
172491	5	410587	13	NULL	NULL	0	NULL	fluorescence response 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The instrument is basically an implementation of the cross-correlation between the excitation source and the induced fluorescence response .
	manualset3
172492	1	410588	13	NULL	NULL	0	NULL	insula	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The insula is the fifth lobe of the brain and it is the least known .
	manualset3
172493	2	410588	13	NULL	NULL	0	NULL	fifth lobe	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The insula is the fifth lobe of the brain and it is the least known .
	manualset3
172494	3	410588	13	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The insula is the fifth lobe of the brain and it is the least known .
	manualset3
172495	1	410589	13	NULL	NULL	0	NULL	total	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 198 patients had a low-energy fracture of the humerus ; 20 of these patients had a shaft fracture ( 10 % ) .
	manualset3
172496	2	410589	13	NULL	NULL	0	NULL	198 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 198 patients had a low-energy fracture of the humerus ; 20 of these patients had a shaft fracture ( 10 % ) .
	manualset3
172497	3	410589	13	NULL	NULL	0	NULL	low-energy fracture	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 198 patients had a low-energy fracture of the humerus ; 20 of these patients had a shaft fracture ( 10 % ) .
	manualset3
172498	4	410589	13	NULL	NULL	0	NULL	humerus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 198 patients had a low-energy fracture of the humerus ; 20 of these patients had a shaft fracture ( 10 % ) .
	manualset3
172499	5	410589	13	NULL	NULL	0	NULL	20	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 198 patients had a low-energy fracture of the humerus ; 20 of these patients had a shaft fracture ( 10 % ) .
	manualset3
172500	6	410589	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 198 patients had a low-energy fracture of the humerus ; 20 of these patients had a shaft fracture ( 10 % ) .
	manualset3
172501	7	410589	13	NULL	NULL	0	NULL	shaft fracture	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 198 patients had a low-energy fracture of the humerus ; 20 of these patients had a shaft fracture ( 10 % ) .
	manualset3
172502	8	410589	13	NULL	NULL	0	NULL	10 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 198 patients had a low-energy fracture of the humerus ; 20 of these patients had a shaft fracture ( 10 % ) .
	manualset3
172503	1	410590	13	NULL	NULL	0	NULL	tumor suppressor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The intact tumor suppressor inhibited all of these .
	manualset3
172621	1	410591	13	NULL	NULL	0	NULL	intensity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The intensity of the head-twitch response and the 5-hydroxytryptamine ( 5-HT ) syndrome ( tremor , fore-paw treading , head-weaving and hind-limb abduction ) was measured in male CFLP mice following IP injection of 5 mg/kg 5-methoxy-N , N-dimethyltryptamine ( 5-MeODMT ) .
	manualset3
172622	2	410591	13	NULL	NULL	0	NULL	head-twitch response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The intensity of the head-twitch response and the 5-hydroxytryptamine ( 5-HT ) syndrome ( tremor , fore-paw treading , head-weaving and hind-limb abduction ) was measured in male CFLP mice following IP injection of 5 mg/kg 5-methoxy-N , N-dimethyltryptamine ( 5-MeODMT ) .
	manualset3
172623	3	410591	13	NULL	NULL	0	NULL	5-hydroxytryptamine ( 5-HT ) syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The intensity of the head-twitch response and the 5-hydroxytryptamine ( 5-HT ) syndrome ( tremor , fore-paw treading , head-weaving and hind-limb abduction ) was measured in male CFLP mice following IP injection of 5 mg/kg 5-methoxy-N , N-dimethyltryptamine ( 5-MeODMT ) .
	manualset3
172624	4	410591	13	NULL	NULL	0	NULL	tremor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The intensity of the head-twitch response and the 5-hydroxytryptamine ( 5-HT ) syndrome ( tremor , fore-paw treading , head-weaving and hind-limb abduction ) was measured in male CFLP mice following IP injection of 5 mg/kg 5-methoxy-N , N-dimethyltryptamine ( 5-MeODMT ) .
	manualset3
172626	5	410591	13	NULL	NULL	0	NULL	hind-limb abduction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The intensity of the head-twitch response and the 5-hydroxytryptamine ( 5-HT ) syndrome ( tremor , fore-paw treading , head-weaving and hind-limb abduction ) was measured in male CFLP mice following IP injection of 5 mg/kg 5-methoxy-N , N-dimethyltryptamine ( 5-MeODMT ) .
	manualset3
172693	6	410591	13	NULL	NULL	0	NULL	male CFLP mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The intensity of the head-twitch response and the 5-hydroxytryptamine ( 5-HT ) syndrome ( tremor , fore-paw treading , head-weaving and hind-limb abduction ) was measured in male CFLP mice following IP injection of 5 mg/kg 5-methoxy-N , N-dimethyltryptamine ( 5-MeODMT ) .
	manualset3
172694	7	410591	13	NULL	NULL	0	NULL	IP injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The intensity of the head-twitch response and the 5-hydroxytryptamine ( 5-HT ) syndrome ( tremor , fore-paw treading , head-weaving and hind-limb abduction ) was measured in male CFLP mice following IP injection of 5 mg/kg 5-methoxy-N , N-dimethyltryptamine ( 5-MeODMT ) .
	manualset3
172695	8	410591	13	NULL	NULL	0	NULL	5 mg/kg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The intensity of the head-twitch response and the 5-hydroxytryptamine ( 5-HT ) syndrome ( tremor , fore-paw treading , head-weaving and hind-limb abduction ) was measured in male CFLP mice following IP injection of 5 mg/kg 5-methoxy-N , N-dimethyltryptamine ( 5-MeODMT ) .
	manualset3
172696	9	410591	13	NULL	NULL	0	NULL	5-methoxy-N , N-dimethyltryptamine ( 5-MeODMT )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The intensity of the head-twitch response and the 5-hydroxytryptamine ( 5-HT ) syndrome ( tremor , fore-paw treading , head-weaving and hind-limb abduction ) was measured in male CFLP mice following IP injection of 5 mg/kg 5-methoxy-N , N-dimethyltryptamine ( 5-MeODMT ) .
	manualset3
172699	1	410592	13	NULL	NULL	0	NULL	intensity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The intensity of the photosensitizer-generated oxidative stress depends on IR-780 release from the effective uptake of polymeric nanocapsules and seems to remain dependent upon the surfactant structure in o/w microemulsion-based templates applied to nanocapsule fabrication .
	manualset3
172700	2	410592	13	NULL	NULL	0	NULL	photosensitizer-generated oxidative stress 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The intensity of the photosensitizer-generated oxidative stress depends on IR-780 release from the effective uptake of polymeric nanocapsules and seems to remain dependent upon the surfactant structure in o/w microemulsion-based templates applied to nanocapsule fabrication .
	manualset3
172701	3	410592	13	NULL	NULL	0	NULL	IR-780 release	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The intensity of the photosensitizer-generated oxidative stress depends on IR-780 release from the effective uptake of polymeric nanocapsules and seems to remain dependent upon the surfactant structure in o/w microemulsion-based templates applied to nanocapsule fabrication .
	manualset3
172702	4	410592	13	NULL	NULL	0	NULL	uptake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The intensity of the photosensitizer-generated oxidative stress depends on IR-780 release from the effective uptake of polymeric nanocapsules and seems to remain dependent upon the surfactant structure in o/w microemulsion-based templates applied to nanocapsule fabrication .
	manualset3
172703	5	410592	13	NULL	NULL	0	NULL	polymeric nanocapsules	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The intensity of the photosensitizer-generated oxidative stress depends on IR-780 release from the effective uptake of polymeric nanocapsules and seems to remain dependent upon the surfactant structure in o/w microemulsion-based templates applied to nanocapsule fabrication .
	manualset3
172704	6	410592	13	NULL	NULL	0	NULL	surfactant structure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The intensity of the photosensitizer-generated oxidative stress depends on IR-780 release from the effective uptake of polymeric nanocapsules and seems to remain dependent upon the surfactant structure in o/w microemulsion-based templates applied to nanocapsule fabrication .
	manualset3
172705	7	410592	13	NULL	NULL	0	NULL	o/w microemulsion-based templates	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The intensity of the photosensitizer-generated oxidative stress depends on IR-780 release from the effective uptake of polymeric nanocapsules and seems to remain dependent upon the surfactant structure in o/w microemulsion-based templates applied to nanocapsule fabrication .
	manualset3
172706	8	410592	13	NULL	NULL	NULL	NULL	nanocapsule 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The intensity of the photosensitizer-generated oxidative stress depends on IR-780 release from the effective uptake of polymeric nanocapsules and seems to remain dependent upon the surfactant structure in o/w microemulsion-based templates applied to nanocapsule fabrication .
	manualset3
172752	9	410592	13	NULL	NULL	0	NULL	fabrication	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The intensity of the photosensitizer-generated oxidative stress depends on IR-780 release from the effective uptake of polymeric nanocapsules and seems to remain dependent upon the surfactant structure in o/w microemulsion-based templates applied to nanocapsule fabrication .
	manualset3
172753	1	410593	13	NULL	NULL	0	NULL	intent	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The intent was to determine whether luxotonic responses , so prominent in striate cortex of primates , are indeed absent in rabbits .
	manualset3
172808	2	410593	13	NULL	NULL	0	NULL	luxotonic responses 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The intent was to determine whether luxotonic responses , so prominent in striate cortex of primates , are indeed absent in rabbits .
	manualset3
172809	3	410593	13	NULL	NULL	0	NULL	striate cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The intent was to determine whether luxotonic responses , so prominent in striate cortex of primates , are indeed absent in rabbits .
	manualset3
172810	4	410593	13	NULL	NULL	0	NULL	primates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The intent was to determine whether luxotonic responses , so prominent in striate cortex of primates , are indeed absent in rabbits .
	manualset3
172811	5	410593	13	NULL	NULL	0	NULL	rabbits	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The intent was to determine whether luxotonic responses , so prominent in striate cortex of primates , are indeed absent in rabbits .
	manualset3
172812	1	410594	13	NULL	NULL	0	NULL	intention	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The intention of the work program was to underwrite the safety , efficacy and ethical aspects of digital practice as well as to protect and add value to the equipment used in radiology .
	manualset3
172813	2	410594	13	NULL	NULL	0	NULL	work program 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The intention of the work program was to underwrite the safety , efficacy and ethical aspects of digital practice as well as to protect and add value to the equipment used in radiology .
	manualset3
172814	3	410594	13	NULL	NULL	0	NULL	safety	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The intention of the work program was to underwrite the safety , efficacy and ethical aspects of digital practice as well as to protect and add value to the equipment used in radiology .
	manualset3
172815	4	410594	13	NULL	NULL	NULL	NULL	efficacy	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The intention of the work program was to underwrite the safety , efficacy and ethical aspects of digital practice as well as to protect and add value to the equipment used in radiology .
	manualset3
172816	5	410594	13	NULL	NULL	0	NULL	ethical aspects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The intention of the work program was to underwrite the safety , efficacy and ethical aspects of digital practice as well as to protect and add value to the equipment used in radiology .
	manualset3
172817	6	410594	13	NULL	NULL	0	NULL	digital practice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The intention of the work program was to underwrite the safety , efficacy and ethical aspects of digital practice as well as to protect and add value to the equipment used in radiology .
	manualset3
172818	7	410594	13	NULL	NULL	0	NULL	value	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The intention of the work program was to underwrite the safety , efficacy and ethical aspects of digital practice as well as to protect and add value to the equipment used in radiology .
	manualset3
172819	8	410594	13	NULL	NULL	0	NULL	equipment	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The intention of the work program was to underwrite the safety , efficacy and ethical aspects of digital practice as well as to protect and add value to the equipment used in radiology .
	manualset3
172820	9	410594	13	NULL	NULL	0	NULL	radiology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The intention of the work program was to underwrite the safety , efficacy and ethical aspects of digital practice as well as to protect and add value to the equipment used in radiology .
	manualset3
172821	1	410595	13	NULL	NULL	0	NULL	interaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction between fully matched DNA and DNA-conjugated polymer was investigated by surface plasmon resonance ( SPR ) technique .
	manualset3
172822	2	410595	13	NULL	NULL	0	NULL	DNA	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction between fully matched DNA and DNA-conjugated polymer was investigated by surface plasmon resonance ( SPR ) technique .
	manualset3
172823	3	410595	13	NULL	NULL	0	NULL	DNA-conjugated polymer 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction between fully matched DNA and DNA-conjugated polymer was investigated by surface plasmon resonance ( SPR ) technique .
	manualset3
172824	4	410595	13	NULL	NULL	0	NULL	surface plasmon resonance ( SPR ) technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction between fully matched DNA and DNA-conjugated polymer was investigated by surface plasmon resonance ( SPR ) technique .
	manualset3
172825	1	410596	13	NULL	NULL	0	NULL	interaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction between human blood-group ( ABO ) substances and enteropathogenic bacterial agents .
	manualset3
172826	2	410596	13	NULL	NULL	NULL	NULL	human blood-group ( ABO ) substances 	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The interaction between human blood-group ( ABO ) substances and enteropathogenic bacterial agents .
	manualset3
172827	3	410596	13	NULL	NULL	0	NULL	enteropathogenic bacterial agents	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction between human blood-group ( ABO ) substances and enteropathogenic bacterial agents .
	manualset3
172828	1	410597	13	NULL	NULL	0	NULL	total	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 201 type 2 diabetic patients on treatment with metformin were enrolled in the study ; pioglitazone was titrated till 45mg/day and glibenclamide till 15mg/day , in association with metformin , respectively .
	manualset3
172829	2	410597	13	NULL	NULL	0	NULL	201 type 2 diabetic patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 201 type 2 diabetic patients on treatment with metformin were enrolled in the study ; pioglitazone was titrated till 45mg/day and glibenclamide till 15mg/day , in association with metformin , respectively .
	manualset3
172830	3	410597	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 201 type 2 diabetic patients on treatment with metformin were enrolled in the study ; pioglitazone was titrated till 45mg/day and glibenclamide till 15mg/day , in association with metformin , respectively .
	manualset3
172831	4	410597	13	NULL	NULL	0	NULL	metformin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 201 type 2 diabetic patients on treatment with metformin were enrolled in the study ; pioglitazone was titrated till 45mg/day and glibenclamide till 15mg/day , in association with metformin , respectively .
	manualset3
172832	5	410597	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 201 type 2 diabetic patients on treatment with metformin were enrolled in the study ; pioglitazone was titrated till 45mg/day and glibenclamide till 15mg/day , in association with metformin , respectively .
	manualset3
172833	6	410597	13	NULL	NULL	0	NULL	pioglitazone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 201 type 2 diabetic patients on treatment with metformin were enrolled in the study ; pioglitazone was titrated till 45mg/day and glibenclamide till 15mg/day , in association with metformin , respectively .
	manualset3
172834	7	410597	13	NULL	NULL	0	NULL	45mg/day	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 201 type 2 diabetic patients on treatment with metformin were enrolled in the study ; pioglitazone was titrated till 45mg/day and glibenclamide till 15mg/day , in association with metformin , respectively .
	manualset3
172835	8	410597	13	NULL	NULL	0	NULL	glibenclamide 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 201 type 2 diabetic patients on treatment with metformin were enrolled in the study ; pioglitazone was titrated till 45mg/day and glibenclamide till 15mg/day , in association with metformin , respectively .
	manualset3
172836	9	410597	13	NULL	NULL	0	NULL	15mg/day	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 201 type 2 diabetic patients on treatment with metformin were enrolled in the study ; pioglitazone was titrated till 45mg/day and glibenclamide till 15mg/day , in association with metformin , respectively .
	manualset3
172837	10	410597	13	NULL	NULL	0	NULL	association 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 201 type 2 diabetic patients on treatment with metformin were enrolled in the study ; pioglitazone was titrated till 45mg/day and glibenclamide till 15mg/day , in association with metformin , respectively .
	manualset3
172838	11	410597	13	NULL	NULL	0	NULL	metformin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 201 type 2 diabetic patients on treatment with metformin were enrolled in the study ; pioglitazone was titrated till 45mg/day and glibenclamide till 15mg/day , in association with metformin , respectively .
	manualset3
172839	1	410598	13	NULL	NULL	0	NULL	interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction between rare-earth ions and DNA from Bashibai sheep was studied by microcalorimetry and electrochemistry .
	manualset3
172840	2	410598	13	NULL	NULL	0	NULL	rare-earth ions 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction between rare-earth ions and DNA from Bashibai sheep was studied by microcalorimetry and electrochemistry .
	manualset3
172841	3	410598	13	NULL	NULL	0	NULL	DNA 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction between rare-earth ions and DNA from Bashibai sheep was studied by microcalorimetry and electrochemistry .
	manualset3
172842	4	410598	13	NULL	NULL	0	NULL	Bashibai sheep	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction between rare-earth ions and DNA from Bashibai sheep was studied by microcalorimetry and electrochemistry .
	manualset3
172843	5	410598	13	NULL	NULL	0	NULL	microcalorimetry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction between rare-earth ions and DNA from Bashibai sheep was studied by microcalorimetry and electrochemistry .
	manualset3
172844	6	410598	13	NULL	NULL	0	NULL	electrochemistry 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction between rare-earth ions and DNA from Bashibai sheep was studied by microcalorimetry and electrochemistry .
	manualset3
172845	1	410599	13	NULL	NULL	0	NULL	interaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction between the nuclear envelope and the cell membrane is expressed by a potential energy function with respect to the distance between them .
	manualset3
172846	2	410599	13	NULL	NULL	0	NULL	nuclear envelope	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction between the nuclear envelope and the cell membrane is expressed by a potential energy function with respect to the distance between them .
	manualset3
172847	3	410599	13	NULL	NULL	0	NULL	cell membrane 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction between the nuclear envelope and the cell membrane is expressed by a potential energy function with respect to the distance between them .
	manualset3
172848	4	410599	13	NULL	NULL	0	NULL	potential energy function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction between the nuclear envelope and the cell membrane is expressed by a potential energy function with respect to the distance between them .
	manualset3
172849	5	410599	13	NULL	NULL	0	NULL	distance	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction between the nuclear envelope and the cell membrane is expressed by a potential energy function with respect to the distance between them .
	manualset3
172850	1	410600	13	NULL	NULL	0	NULL	interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction between the platinum ( II ) complexes and pET22b plasmid DNA was observed by agarose gel electrophoresis , revealing that complex 2f has the capacity to distort plasmid DNA in a manner distinct from that of oxaliplatin .
	manualset3
172851	2	410600	13	NULL	NULL	0	NULL	platinum ( II ) complexes 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction between the platinum ( II ) complexes and pET22b plasmid DNA was observed by agarose gel electrophoresis , revealing that complex 2f has the capacity to distort plasmid DNA in a manner distinct from that of oxaliplatin .
	manualset3
172852	3	410600	13	NULL	NULL	0	NULL	pET22b plasmid DNA	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction between the platinum ( II ) complexes and pET22b plasmid DNA was observed by agarose gel electrophoresis , revealing that complex 2f has the capacity to distort plasmid DNA in a manner distinct from that of oxaliplatin .
	manualset3
172853	4	410600	13	NULL	NULL	0	NULL	agarose gel electrophoresis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction between the platinum ( II ) complexes and pET22b plasmid DNA was observed by agarose gel electrophoresis , revealing that complex 2f has the capacity to distort plasmid DNA in a manner distinct from that of oxaliplatin .
	manualset3
172854	5	410600	13	NULL	NULL	0	NULL	complex 2f 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction between the platinum ( II ) complexes and pET22b plasmid DNA was observed by agarose gel electrophoresis , revealing that complex 2f has the capacity to distort plasmid DNA in a manner distinct from that of oxaliplatin .
	manualset3
172855	6	410600	13	NULL	NULL	0	NULL	capacity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction between the platinum ( II ) complexes and pET22b plasmid DNA was observed by agarose gel electrophoresis , revealing that complex 2f has the capacity to distort plasmid DNA in a manner distinct from that of oxaliplatin .
	manualset3
172856	7	410600	13	NULL	NULL	0	NULL	plasmid DNA	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction between the platinum ( II ) complexes and pET22b plasmid DNA was observed by agarose gel electrophoresis , revealing that complex 2f has the capacity to distort plasmid DNA in a manner distinct from that of oxaliplatin .
	manualset3
172857	8	410600	13	NULL	NULL	0	NULL	oxaliplatin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction between the platinum ( II ) complexes and pET22b plasmid DNA was observed by agarose gel electrophoresis , revealing that complex 2f has the capacity to distort plasmid DNA in a manner distinct from that of oxaliplatin .
	manualset3
172858	1	410601	13	NULL	NULL	0	NULL	interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction between yeast inorganic pyrophosphatase and the simplest organic substrate , methylpyrophosphate , was studied .
	manualset3
172859	2	410601	13	NULL	NULL	0	NULL	yeast inorganic pyrophosphatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction between yeast inorganic pyrophosphatase and the simplest organic substrate , methylpyrophosphate , was studied .
	manualset3
172860	3	410601	13	NULL	NULL	0	NULL	organic substrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction between yeast inorganic pyrophosphatase and the simplest organic substrate , methylpyrophosphate , was studied .
	manualset3
172861	4	410601	13	NULL	NULL	0	NULL	methylpyrophosphate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction between yeast inorganic pyrophosphatase and the simplest organic substrate , methylpyrophosphate , was studied .
	manualset3
172862	1	410602	13	NULL	NULL	0	NULL	interaction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of high BAS and high Behavioral Inhibition System ( BIS ) sensitivities also predicted greater likelihood of progression to bipolar I. We discuss implications of the findings for the bipolar spectrum concept , the BAS model of bipolar disorder , and early intervention efforts .
	manualset3
172863	2	410602	13	NULL	NULL	NULL	NULL	high BAS sensitivities 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The interaction of high BAS and high Behavioral Inhibition System ( BIS ) sensitivities also predicted greater likelihood of progression to bipolar I. We discuss implications of the findings for the bipolar spectrum concept , the BAS model of bipolar disorder , and early intervention efforts .
	manualset3
172864	3	410602	13	NULL	NULL	0	NULL	high Behavioral Inhibition System ( BIS ) sensitivities 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of high BAS and high Behavioral Inhibition System ( BIS ) sensitivities also predicted greater likelihood of progression to bipolar I. We discuss implications of the findings for the bipolar spectrum concept , the BAS model of bipolar disorder , and early intervention efforts .
	manualset3
172865	4	410602	13	NULL	NULL	0	NULL	likelihood 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of high BAS and high Behavioral Inhibition System ( BIS ) sensitivities also predicted greater likelihood of progression to bipolar I. We discuss implications of the findings for the bipolar spectrum concept , the BAS model of bipolar disorder , and early intervention efforts .
	manualset3
172866	5	410602	13	NULL	NULL	0	NULL	progression 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of high BAS and high Behavioral Inhibition System ( BIS ) sensitivities also predicted greater likelihood of progression to bipolar I. We discuss implications of the findings for the bipolar spectrum concept , the BAS model of bipolar disorder , and early intervention efforts .
	manualset3
172867	6	410602	13	NULL	NULL	NULL	NULL	bipolar I	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The interaction of high BAS and high Behavioral Inhibition System ( BIS ) sensitivities also predicted greater likelihood of progression to bipolar I. We discuss implications of the findings for the bipolar spectrum concept , the BAS model of bipolar disorder , and early intervention efforts .
	manualset3
172868	7	410602	13	NULL	NULL	0	NULL	implications 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of high BAS and high Behavioral Inhibition System ( BIS ) sensitivities also predicted greater likelihood of progression to bipolar I. We discuss implications of the findings for the bipolar spectrum concept , the BAS model of bipolar disorder , and early intervention efforts .
	manualset3
172869	8	410602	13	NULL	NULL	0	NULL	findings 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of high BAS and high Behavioral Inhibition System ( BIS ) sensitivities also predicted greater likelihood of progression to bipolar I. We discuss implications of the findings for the bipolar spectrum concept , the BAS model of bipolar disorder , and early intervention efforts .
	manualset3
172870	9	410602	13	NULL	NULL	0	NULL	bipolar spectrum concept	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of high BAS and high Behavioral Inhibition System ( BIS ) sensitivities also predicted greater likelihood of progression to bipolar I. We discuss implications of the findings for the bipolar spectrum concept , the BAS model of bipolar disorder , and early intervention efforts .
	manualset3
172871	10	410602	13	NULL	NULL	0	NULL	BAS model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of high BAS and high Behavioral Inhibition System ( BIS ) sensitivities also predicted greater likelihood of progression to bipolar I. We discuss implications of the findings for the bipolar spectrum concept , the BAS model of bipolar disorder , and early intervention efforts .
	manualset3
172872	11	410602	13	NULL	NULL	NULL	NULL	bipolar disorder 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The interaction of high BAS and high Behavioral Inhibition System ( BIS ) sensitivities also predicted greater likelihood of progression to bipolar I. We discuss implications of the findings for the bipolar spectrum concept , the BAS model of bipolar disorder , and early intervention efforts .
	manualset3
172873	12	410602	13	NULL	NULL	0	NULL	intervention efforts	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of high BAS and high Behavioral Inhibition System ( BIS ) sensitivities also predicted greater likelihood of progression to bipolar I. We discuss implications of the findings for the bipolar spectrum concept , the BAS model of bipolar disorder , and early intervention efforts .
	manualset3
172874	1	410603	13	NULL	NULL	0	NULL	interaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of insulin with human circulating granulocytes was studied with the use of 125I-insulin .
	manualset3
172875	2	410603	13	NULL	NULL	0	NULL	insulin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of insulin with human circulating granulocytes was studied with the use of 125I-insulin .
	manualset3
172876	3	410603	13	NULL	NULL	0	NULL	 human circulating granulocytes 	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of insulin with human circulating granulocytes was studied with the use of 125I-insulin .
	manualset3
172877	4	410603	13	NULL	NULL	0	NULL	use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of insulin with human circulating granulocytes was studied with the use of 125I-insulin .
	manualset3
172878	5	410603	13	NULL	NULL	0	NULL	125I-insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of insulin with human circulating granulocytes was studied with the use of 125I-insulin .
	manualset3
172879	1	410604	13	NULL	NULL	0	NULL	interaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of labeled fibronectin and the labeled , gelatin-binding domain of fibronectin with cells after fractionation on polyacrylamide gels indicated that GP170 is the primary procollagen receptor for fibronectin in the extracellular matrix .
	manualset3
172880	2	410604	13	NULL	NULL	0	NULL	fibronectin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of labeled fibronectin and the labeled , gelatin-binding domain of fibronectin with cells after fractionation on polyacrylamide gels indicated that GP170 is the primary procollagen receptor for fibronectin in the extracellular matrix .
	manualset3
172881	3	410604	13	NULL	NULL	0	NULL	gelatin-binding domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of labeled fibronectin and the labeled , gelatin-binding domain of fibronectin with cells after fractionation on polyacrylamide gels indicated that GP170 is the primary procollagen receptor for fibronectin in the extracellular matrix .
	manualset3
172882	4	410604	13	NULL	NULL	0	NULL	fibronectin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of labeled fibronectin and the labeled , gelatin-binding domain of fibronectin with cells after fractionation on polyacrylamide gels indicated that GP170 is the primary procollagen receptor for fibronectin in the extracellular matrix .
	manualset3
172883	5	410604	13	NULL	NULL	0	NULL	cells 	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of labeled fibronectin and the labeled , gelatin-binding domain of fibronectin with cells after fractionation on polyacrylamide gels indicated that GP170 is the primary procollagen receptor for fibronectin in the extracellular matrix .
	manualset3
172884	6	410604	13	NULL	NULL	0	NULL	fractionation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of labeled fibronectin and the labeled , gelatin-binding domain of fibronectin with cells after fractionation on polyacrylamide gels indicated that GP170 is the primary procollagen receptor for fibronectin in the extracellular matrix .
	manualset3
172885	7	410604	13	NULL	NULL	0	NULL	polyacrylamide gels	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of labeled fibronectin and the labeled , gelatin-binding domain of fibronectin with cells after fractionation on polyacrylamide gels indicated that GP170 is the primary procollagen receptor for fibronectin in the extracellular matrix .
	manualset3
172886	8	410604	13	NULL	NULL	0	NULL	GP170 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of labeled fibronectin and the labeled , gelatin-binding domain of fibronectin with cells after fractionation on polyacrylamide gels indicated that GP170 is the primary procollagen receptor for fibronectin in the extracellular matrix .
	manualset3
172887	9	410604	13	NULL	NULL	0	NULL	primary procollagen receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of labeled fibronectin and the labeled , gelatin-binding domain of fibronectin with cells after fractionation on polyacrylamide gels indicated that GP170 is the primary procollagen receptor for fibronectin in the extracellular matrix .
	manualset3
172888	10	410604	13	NULL	NULL	0	NULL	fibronectin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of labeled fibronectin and the labeled , gelatin-binding domain of fibronectin with cells after fractionation on polyacrylamide gels indicated that GP170 is the primary procollagen receptor for fibronectin in the extracellular matrix .
	manualset3
172889	11	410604	13	NULL	NULL	0	NULL	extracellular matrix	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of labeled fibronectin and the labeled , gelatin-binding domain of fibronectin with cells after fractionation on polyacrylamide gels indicated that GP170 is the primary procollagen receptor for fibronectin in the extracellular matrix .
	manualset3
172890	1	410605	13	NULL	NULL	0	NULL	interaction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of liposomes with a series of fluorescent berberine derivatives having different alkyl chain lengths has been investigated .
	manualset3
172891	2	410605	13	NULL	NULL	0	NULL	liposomes 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of liposomes with a series of fluorescent berberine derivatives having different alkyl chain lengths has been investigated .
	manualset3
172892	3	410605	13	NULL	NULL	0	NULL	series 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of liposomes with a series of fluorescent berberine derivatives having different alkyl chain lengths has been investigated .
	manualset3
172893	4	410605	13	NULL	NULL	0	NULL	fluorescent berberine derivatives 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of liposomes with a series of fluorescent berberine derivatives having different alkyl chain lengths has been investigated .
	manualset3
172894	5	410605	13	NULL	NULL	0	NULL	alkyl chain lengths 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of liposomes with a series of fluorescent berberine derivatives having different alkyl chain lengths has been investigated .
	manualset3
172895	1	410606	13	NULL	NULL	0	NULL	interaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of these ionized aminothiols with phosphate groups of DNA is essentially an electrostatic one , like that for metallic cations , and can be expressed by the Schildkraut-Lifson equation Tm = a log Cradio + b , where a and b are adjustable parameters and Cradio is the concentration of the radioprotectors .
	manualset3
172896	2	410606	13	NULL	NULL	0	NULL	ionized aminothiols	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of these ionized aminothiols with phosphate groups of DNA is essentially an electrostatic one , like that for metallic cations , and can be expressed by the Schildkraut-Lifson equation Tm = a log Cradio + b , where a and b are adjustable parameters and Cradio is the concentration of the radioprotectors .
	manualset3
172897	3	410606	13	NULL	NULL	0	NULL	phosphate groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of these ionized aminothiols with phosphate groups of DNA is essentially an electrostatic one , like that for metallic cations , and can be expressed by the Schildkraut-Lifson equation Tm = a log Cradio + b , where a and b are adjustable parameters and Cradio is the concentration of the radioprotectors .
	manualset3
172898	4	410606	13	NULL	NULL	0	NULL	DNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of these ionized aminothiols with phosphate groups of DNA is essentially an electrostatic one , like that for metallic cations , and can be expressed by the Schildkraut-Lifson equation Tm = a log Cradio + b , where a and b are adjustable parameters and Cradio is the concentration of the radioprotectors .
	manualset3
172899	5	410606	13	NULL	NULL	0	NULL	metallic cations 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of these ionized aminothiols with phosphate groups of DNA is essentially an electrostatic one , like that for metallic cations , and can be expressed by the Schildkraut-Lifson equation Tm = a log Cradio + b , where a and b are adjustable parameters and Cradio is the concentration of the radioprotectors .
	manualset3
172900	6	410606	13	NULL	NULL	0	NULL	Schildkraut-Lifson equation Tm = a log Cradio + b 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of these ionized aminothiols with phosphate groups of DNA is essentially an electrostatic one , like that for metallic cations , and can be expressed by the Schildkraut-Lifson equation Tm = a log Cradio + b , where a and b are adjustable parameters and Cradio is the concentration of the radioprotectors .
	manualset3
172901	7	410606	13	NULL	NULL	0	NULL	parameters 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of these ionized aminothiols with phosphate groups of DNA is essentially an electrostatic one , like that for metallic cations , and can be expressed by the Schildkraut-Lifson equation Tm = a log Cradio + b , where a and b are adjustable parameters and Cradio is the concentration of the radioprotectors .
	manualset3
172902	8	410606	13	NULL	NULL	0	NULL	Cradio 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of these ionized aminothiols with phosphate groups of DNA is essentially an electrostatic one , like that for metallic cations , and can be expressed by the Schildkraut-Lifson equation Tm = a log Cradio + b , where a and b are adjustable parameters and Cradio is the concentration of the radioprotectors .
	manualset3
172903	9	410606	13	NULL	NULL	0	NULL	concentration 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of these ionized aminothiols with phosphate groups of DNA is essentially an electrostatic one , like that for metallic cations , and can be expressed by the Schildkraut-Lifson equation Tm = a log Cradio + b , where a and b are adjustable parameters and Cradio is the concentration of the radioprotectors .
	manualset3
172904	10	410606	13	NULL	NULL	0	NULL	radioprotectors 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The interaction of these ionized aminothiols with phosphate groups of DNA is essentially an electrostatic one , like that for metallic cations , and can be expressed by the Schildkraut-Lifson equation Tm = a log Cradio + b , where a and b are adjustable parameters and Cradio is the concentration of the radioprotectors .
	manualset3
172905	1	410607	13	NULL	NULL	0	NULL	total 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 213 strains of lactic acid bacteria were examined in this study .
	manualset3
172906	2	410607	13	NULL	NULL	0	NULL	213 strains 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 213 strains of lactic acid bacteria were examined in this study .
	manualset3
172907	3	410607	13	NULL	NULL	0	NULL	lactic acid bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 213 strains of lactic acid bacteria were examined in this study .
	manualset3
172908	4	410607	13	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 213 strains of lactic acid bacteria were examined in this study .
	manualset3
172909	1	410608	13	NULL	NULL	0	NULL	interassay CV 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The interassay CV was 9.9 % and the intra-assay CV 7.2 % .
	manualset3
172910	2	410608	13	NULL	NULL	0	NULL	9.9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The interassay CV was 9.9 % and the intra-assay CV 7.2 % .
	manualset3
172911	3	410608	13	NULL	NULL	0	NULL	 intra-assay CV	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The interassay CV was 9.9 % and the intra-assay CV 7.2 % .
	manualset3
172912	4	410608	13	NULL	NULL	0	NULL	7.2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The interassay CV was 9.9 % and the intra-assay CV 7.2 % .
	manualset3
172913	1	410609	13	NULL	NULL	0	NULL	interest 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The interest in the limit of viability originated from various sources , including legal requirements , the rejection of mechnical life support , competition for resources , concerns about handicaps , and proximity to the fetus with its limited rights .
	manualset3
172914	2	410609	13	NULL	NULL	0	NULL	limit of viability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The interest in the limit of viability originated from various sources , including legal requirements , the rejection of mechnical life support , competition for resources , concerns about handicaps , and proximity to the fetus with its limited rights .
	manualset3
172915	3	410609	13	NULL	NULL	0	NULL	various sources	NamedEntity 												NULL		0	NULL	NULL	NULL	NULL	NULL	The interest in the limit of viability originated from various sources , including legal requirements , the rejection of mechnical life support , competition for resources , concerns about handicaps , and proximity to the fetus with its limited rights .
	manualset3
172916	4	410609	13	NULL	NULL	0	NULL	legal requirements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The interest in the limit of viability originated from various sources , including legal requirements , the rejection of mechnical life support , competition for resources , concerns about handicaps , and proximity to the fetus with its limited rights .
	manualset3
172917	5	410609	13	NULL	NULL	0	NULL	rejection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The interest in the limit of viability originated from various sources , including legal requirements , the rejection of mechnical life support , competition for resources , concerns about handicaps , and proximity to the fetus with its limited rights .
	manualset3
172918	6	410609	13	NULL	NULL	0	NULL	mechnical life support	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The interest in the limit of viability originated from various sources , including legal requirements , the rejection of mechnical life support , competition for resources , concerns about handicaps , and proximity to the fetus with its limited rights .
	manualset3
172919	7	410609	13	NULL	NULL	0	NULL	competition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The interest in the limit of viability originated from various sources , including legal requirements , the rejection of mechnical life support , competition for resources , concerns about handicaps , and proximity to the fetus with its limited rights .
	manualset3
172920	8	410609	13	NULL	NULL	0	NULL	resources 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The interest in the limit of viability originated from various sources , including legal requirements , the rejection of mechnical life support , competition for resources , concerns about handicaps , and proximity to the fetus with its limited rights .
	manualset3
172921	9	410609	13	NULL	NULL	0	NULL	concerns 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The interest in the limit of viability originated from various sources , including legal requirements , the rejection of mechnical life support , competition for resources , concerns about handicaps , and proximity to the fetus with its limited rights .
	manualset3
172922	10	410609	13	NULL	NULL	0	NULL	handicaps 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The interest in the limit of viability originated from various sources , including legal requirements , the rejection of mechnical life support , competition for resources , concerns about handicaps , and proximity to the fetus with its limited rights .
	manualset3
172923	11	410609	13	NULL	NULL	0	NULL	fetus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The interest in the limit of viability originated from various sources , including legal requirements , the rejection of mechnical life support , competition for resources , concerns about handicaps , and proximity to the fetus with its limited rights .
	manualset3
172924	12	410609	13	NULL	NULL	0	NULL	rights 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The interest in the limit of viability originated from various sources , including legal requirements , the rejection of mechnical life support , competition for resources , concerns about handicaps , and proximity to the fetus with its limited rights .
	manualset3
172925	1	410610	13	NULL	NULL	0	NULL	interest 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The interest of this case lies in the rarity of amyloidosis localisation and in the uncommon clinical presentation as acute cholecystitis .
	manualset3
172926	2	410610	13	NULL	NULL	0	NULL	case 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The interest of this case lies in the rarity of amyloidosis localisation and in the uncommon clinical presentation as acute cholecystitis .
	manualset3
172927	3	410610	13	NULL	NULL	0	NULL	rarity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The interest of this case lies in the rarity of amyloidosis localisation and in the uncommon clinical presentation as acute cholecystitis .
	manualset3
172928	4	410610	13	NULL	NULL	0	NULL	amyloidosis localisation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The interest of this case lies in the rarity of amyloidosis localisation and in the uncommon clinical presentation as acute cholecystitis .
	manualset3
172929	5	410610	13	NULL	NULL	0	NULL	clinical presentation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The interest of this case lies in the rarity of amyloidosis localisation and in the uncommon clinical presentation as acute cholecystitis .
	manualset3
172930	6	410610	13	NULL	NULL	0	NULL	acute cholecystitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The interest of this case lies in the rarity of amyloidosis localisation and in the uncommon clinical presentation as acute cholecystitis .
	manualset3
172931	1	410611	13	NULL	NULL	0	NULL	interferometric optical Fourier processor	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The interferometric optical Fourier processor is demonstrated in a moving-object trajectory estimation system .
	manualset3
172932	2	410611	13	NULL	NULL	0	NULL	moving-object trajectory estimation system	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The interferometric optical Fourier processor is demonstrated in a moving-object trajectory estimation system .
	manualset3
172933	1	410612	13	NULL	NULL	0	NULL	allylboronate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The intermediate allylboronate was oxidized to the stereodefined allylic 1 , 4-diol .
	manualset3
172934	2	410612	13	NULL	NULL	0	NULL	stereodefined allylic 1 , 4-diol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The intermediate allylboronate was oxidized to the stereodefined allylic 1 , 4-diol .
	manualset3
172935	1	410613	13	NULL	NULL	0	NULL	lipoprotein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The intermediate lipoprotein was relatively rich in apoprotein B , apoprotein VS-2 , cholesterol , and phospholipids and poor in triglycerides and apoprotein C. The mean diameter of intermediate lipoprotein was 269 A ( compared with 427 A , the mean Sf rate was 30.5 ( compared with 115 ) , and the mean weight was 7.0 X 10 ( 6 ) daltons ( compared with 23.1 X 10 ( 6 ) ) .
	manualset3
172936	2	410613	13	NULL	NULL	0	NULL	apoprotein B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The intermediate lipoprotein was relatively rich in apoprotein B , apoprotein VS-2 , cholesterol , and phospholipids and poor in triglycerides and apoprotein C. The mean diameter of intermediate lipoprotein was 269 A ( compared with 427 A , the mean Sf rate was 30.5 ( compared with 115 ) , and the mean weight was 7.0 X 10 ( 6 ) daltons ( compared with 23.1 X 10 ( 6 ) ) .
	manualset3
172937	3	410613	13	NULL	NULL	0	NULL	apoprotein VS-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The intermediate lipoprotein was relatively rich in apoprotein B , apoprotein VS-2 , cholesterol , and phospholipids and poor in triglycerides and apoprotein C. The mean diameter of intermediate lipoprotein was 269 A ( compared with 427 A , the mean Sf rate was 30.5 ( compared with 115 ) , and the mean weight was 7.0 X 10 ( 6 ) daltons ( compared with 23.1 X 10 ( 6 ) ) .
	manualset3
172938	4	410613	13	NULL	NULL	0	NULL	cholesterol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The intermediate lipoprotein was relatively rich in apoprotein B , apoprotein VS-2 , cholesterol , and phospholipids and poor in triglycerides and apoprotein C. The mean diameter of intermediate lipoprotein was 269 A ( compared with 427 A , the mean Sf rate was 30.5 ( compared with 115 ) , and the mean weight was 7.0 X 10 ( 6 ) daltons ( compared with 23.1 X 10 ( 6 ) ) .
	manualset3
172939	5	410613	13	NULL	NULL	0	NULL	phospholipids 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The intermediate lipoprotein was relatively rich in apoprotein B , apoprotein VS-2 , cholesterol , and phospholipids and poor in triglycerides and apoprotein C. The mean diameter of intermediate lipoprotein was 269 A ( compared with 427 A , the mean Sf rate was 30.5 ( compared with 115 ) , and the mean weight was 7.0 X 10 ( 6 ) daltons ( compared with 23.1 X 10 ( 6 ) ) .
	manualset3
172940	6	410613	13	NULL	NULL	0	NULL	triglycerides 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The intermediate lipoprotein was relatively rich in apoprotein B , apoprotein VS-2 , cholesterol , and phospholipids and poor in triglycerides and apoprotein C. The mean diameter of intermediate lipoprotein was 269 A ( compared with 427 A , the mean Sf rate was 30.5 ( compared with 115 ) , and the mean weight was 7.0 X 10 ( 6 ) daltons ( compared with 23.1 X 10 ( 6 ) ) .
	manualset3
172941	7	410613	13	NULL	NULL	0	NULL	apoprotein C	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The intermediate lipoprotein was relatively rich in apoprotein B , apoprotein VS-2 , cholesterol , and phospholipids and poor in triglycerides and apoprotein C. The mean diameter of intermediate lipoprotein was 269 A ( compared with 427 A , the mean Sf rate was 30.5 ( compared with 115 ) , and the mean weight was 7.0 X 10 ( 6 ) daltons ( compared with 23.1 X 10 ( 6 ) ) .
	manualset3
172942	8	410613	13	NULL	NULL	0	NULL	diameter 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The intermediate lipoprotein was relatively rich in apoprotein B , apoprotein VS-2 , cholesterol , and phospholipids and poor in triglycerides and apoprotein C. The mean diameter of intermediate lipoprotein was 269 A ( compared with 427 A , the mean Sf rate was 30.5 ( compared with 115 ) , and the mean weight was 7.0 X 10 ( 6 ) daltons ( compared with 23.1 X 10 ( 6 ) ) .
	manualset3
172943	9	410613	13	NULL	NULL	0	NULL	lipoprotein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The intermediate lipoprotein was relatively rich in apoprotein B , apoprotein VS-2 , cholesterol , and phospholipids and poor in triglycerides and apoprotein C. The mean diameter of intermediate lipoprotein was 269 A ( compared with 427 A , the mean Sf rate was 30.5 ( compared with 115 ) , and the mean weight was 7.0 X 10 ( 6 ) daltons ( compared with 23.1 X 10 ( 6 ) ) .
	manualset3
172944	10	410613	13	NULL	NULL	0	NULL	269 A	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The intermediate lipoprotein was relatively rich in apoprotein B , apoprotein VS-2 , cholesterol , and phospholipids and poor in triglycerides and apoprotein C. The mean diameter of intermediate lipoprotein was 269 A ( compared with 427 A , the mean Sf rate was 30.5 ( compared with 115 ) , and the mean weight was 7.0 X 10 ( 6 ) daltons ( compared with 23.1 X 10 ( 6 ) ) .
	manualset3
172945	11	410613	13	NULL	NULL	0	NULL	427 A	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The intermediate lipoprotein was relatively rich in apoprotein B , apoprotein VS-2 , cholesterol , and phospholipids and poor in triglycerides and apoprotein C. The mean diameter of intermediate lipoprotein was 269 A ( compared with 427 A , the mean Sf rate was 30.5 ( compared with 115 ) , and the mean weight was 7.0 X 10 ( 6 ) daltons ( compared with 23.1 X 10 ( 6 ) ) .
	manualset3
172946	12	410613	13	NULL	NULL	0	NULL	mean Sf rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The intermediate lipoprotein was relatively rich in apoprotein B , apoprotein VS-2 , cholesterol , and phospholipids and poor in triglycerides and apoprotein C. The mean diameter of intermediate lipoprotein was 269 A ( compared with 427 A , the mean Sf rate was 30.5 ( compared with 115 ) , and the mean weight was 7.0 X 10 ( 6 ) daltons ( compared with 23.1 X 10 ( 6 ) ) .
	manualset3
172947	13	410613	13	NULL	NULL	0	NULL	30.5 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The intermediate lipoprotein was relatively rich in apoprotein B , apoprotein VS-2 , cholesterol , and phospholipids and poor in triglycerides and apoprotein C. The mean diameter of intermediate lipoprotein was 269 A ( compared with 427 A , the mean Sf rate was 30.5 ( compared with 115 ) , and the mean weight was 7.0 X 10 ( 6 ) daltons ( compared with 23.1 X 10 ( 6 ) ) .
	manualset3
172948	14	410613	13	NULL	NULL	0	NULL	115 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The intermediate lipoprotein was relatively rich in apoprotein B , apoprotein VS-2 , cholesterol , and phospholipids and poor in triglycerides and apoprotein C. The mean diameter of intermediate lipoprotein was 269 A ( compared with 427 A , the mean Sf rate was 30.5 ( compared with 115 ) , and the mean weight was 7.0 X 10 ( 6 ) daltons ( compared with 23.1 X 10 ( 6 ) ) .
	manualset3
172949	15	410613	13	NULL	NULL	0	NULL	mean weight 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The intermediate lipoprotein was relatively rich in apoprotein B , apoprotein VS-2 , cholesterol , and phospholipids and poor in triglycerides and apoprotein C. The mean diameter of intermediate lipoprotein was 269 A ( compared with 427 A , the mean Sf rate was 30.5 ( compared with 115 ) , and the mean weight was 7.0 X 10 ( 6 ) daltons ( compared with 23.1 X 10 ( 6 ) ) .
	manualset3
172950	16	410613	13	NULL	NULL	0	NULL	7.0 X 10 ( 6 ) daltons	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The intermediate lipoprotein was relatively rich in apoprotein B , apoprotein VS-2 , cholesterol , and phospholipids and poor in triglycerides and apoprotein C. The mean diameter of intermediate lipoprotein was 269 A ( compared with 427 A , the mean Sf rate was 30.5 ( compared with 115 ) , and the mean weight was 7.0 X 10 ( 6 ) daltons ( compared with 23.1 X 10 ( 6 ) ) .
	manualset3
172951	17	410613	13	NULL	NULL	0	NULL	23.1 X 10 ( 6 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The intermediate lipoprotein was relatively rich in apoprotein B , apoprotein VS-2 , cholesterol , and phospholipids and poor in triglycerides and apoprotein C. The mean diameter of intermediate lipoprotein was 269 A ( compared with 427 A , the mean Sf rate was 30.5 ( compared with 115 ) , and the mean weight was 7.0 X 10 ( 6 ) daltons ( compared with 23.1 X 10 ( 6 ) ) .
	manualset3
172952	1	410614	13	NULL	NULL	0	NULL	internal organization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The internal organization of the muscle cell is dictated by the necessary regular arrangement of repeated units within the protein myofibrils that mediate muscle contraction .
	manualset3
172953	2	410614	13	NULL	NULL	0	NULL	muscle cell 	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The internal organization of the muscle cell is dictated by the necessary regular arrangement of repeated units within the protein myofibrils that mediate muscle contraction .
	manualset3
172954	3	410614	13	NULL	NULL	0	NULL	arrangement 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The internal organization of the muscle cell is dictated by the necessary regular arrangement of repeated units within the protein myofibrils that mediate muscle contraction .
	manualset3
172955	4	410614	13	NULL	NULL	0	NULL	units 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The internal organization of the muscle cell is dictated by the necessary regular arrangement of repeated units within the protein myofibrils that mediate muscle contraction .
	manualset3
172956	5	410614	13	NULL	NULL	0	NULL	protein myofibrils	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The internal organization of the muscle cell is dictated by the necessary regular arrangement of repeated units within the protein myofibrils that mediate muscle contraction .
	manualset3
172957	6	410614	13	NULL	NULL	0	NULL	muscle contraction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The internal organization of the muscle cell is dictated by the necessary regular arrangement of repeated units within the protein myofibrils that mediate muscle contraction .
	manualset3
172958	1	410615	13	NULL	NULL	0	NULL	internet 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The internet as a setting for mental health service utilisation by young people .
	manualset3
172959	2	410615	13	NULL	NULL	0	NULL	setting 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The internet as a setting for mental health service utilisation by young people .
	manualset3
172960	3	410615	13	NULL	NULL	0	NULL	mental health service	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The internet as a setting for mental health service utilisation by young people .
	manualset3
172961	4	410615	13	NULL	NULL	0	NULL	utilisation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The internet as a setting for mental health service utilisation by young people .
	manualset3
172962	5	410615	13	NULL	NULL	0	NULL	young people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The internet as a setting for mental health service utilisation by young people .
	manualset3
172963	1	410616	13	NULL	NULL	0	NULL	agreement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The interobserver agreement in the detection of lesions was analyzed .
	manualset3
172964	2	410616	13	NULL	NULL	0	NULL	detection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The interobserver agreement in the detection of lesions was analyzed .
	manualset3
172965	3	410616	13	NULL	NULL	0	NULL	lesions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The interobserver agreement in the detection of lesions was analyzed .
	manualset3
172966	1	410617	13	NULL	NULL	NULL	NULL	interpretation 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The interpretation of economic analyses of phase III clinical trials raises issues related to the perspective of the investigators , study design , collection of data on resource utilization , learning curve effects and generalizability of the results to other settings .
	manualset3
172967	2	410617	13	NULL	NULL	0	NULL	economic analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of economic analyses of phase III clinical trials raises issues related to the perspective of the investigators , study design , collection of data on resource utilization , learning curve effects and generalizability of the results to other settings .
	manualset3
172968	3	410617	13	NULL	NULL	0	NULL	 phase III clinical trials	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of economic analyses of phase III clinical trials raises issues related to the perspective of the investigators , study design , collection of data on resource utilization , learning curve effects and generalizability of the results to other settings .
	manualset3
172969	4	410617	13	NULL	NULL	0	NULL	issues 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of economic analyses of phase III clinical trials raises issues related to the perspective of the investigators , study design , collection of data on resource utilization , learning curve effects and generalizability of the results to other settings .
	manualset3
172970	5	410617	13	NULL	NULL	0	NULL	perspective 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of economic analyses of phase III clinical trials raises issues related to the perspective of the investigators , study design , collection of data on resource utilization , learning curve effects and generalizability of the results to other settings .
	manualset3
172971	6	410617	13	NULL	NULL	0	NULL	investigators 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of economic analyses of phase III clinical trials raises issues related to the perspective of the investigators , study design , collection of data on resource utilization , learning curve effects and generalizability of the results to other settings .
	manualset3
172972	7	410617	13	NULL	NULL	0	NULL	study design	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of economic analyses of phase III clinical trials raises issues related to the perspective of the investigators , study design , collection of data on resource utilization , learning curve effects and generalizability of the results to other settings .
	manualset3
172973	8	410617	13	NULL	NULL	0	NULL	collection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of economic analyses of phase III clinical trials raises issues related to the perspective of the investigators , study design , collection of data on resource utilization , learning curve effects and generalizability of the results to other settings .
	manualset3
172974	9	410617	13	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of economic analyses of phase III clinical trials raises issues related to the perspective of the investigators , study design , collection of data on resource utilization , learning curve effects and generalizability of the results to other settings .
	manualset3
172975	10	410617	13	NULL	NULL	0	NULL	resource utilization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of economic analyses of phase III clinical trials raises issues related to the perspective of the investigators , study design , collection of data on resource utilization , learning curve effects and generalizability of the results to other settings .
	manualset3
172976	11	410617	13	NULL	NULL	0	NULL	learning curve effects	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of economic analyses of phase III clinical trials raises issues related to the perspective of the investigators , study design , collection of data on resource utilization , learning curve effects and generalizability of the results to other settings .
	manualset3
172977	12	410617	13	NULL	NULL	0	NULL	generalizability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of economic analyses of phase III clinical trials raises issues related to the perspective of the investigators , study design , collection of data on resource utilization , learning curve effects and generalizability of the results to other settings .
	manualset3
172978	13	410617	13	NULL	NULL	0	NULL	results 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of economic analyses of phase III clinical trials raises issues related to the perspective of the investigators , study design , collection of data on resource utilization , learning curve effects and generalizability of the results to other settings .
	manualset3
172979	14	410617	13	NULL	NULL	0	NULL	settings 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of economic analyses of phase III clinical trials raises issues related to the perspective of the investigators , study design , collection of data on resource utilization , learning curve effects and generalizability of the results to other settings .
	manualset3
172980	1	410618	13	NULL	NULL	NULL	NULL	interpretation 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The interpretation of findings is that Black-White differences reflect both macro-historical change and the microlevel community experiences of young people .
	manualset3
172981	2	410618	13	NULL	NULL	0	NULL	findings 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of findings is that Black-White differences reflect both macro-historical change and the microlevel community experiences of young people .
	manualset3
172982	3	410618	13	NULL	NULL	0	NULL	Black-White differences	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of findings is that Black-White differences reflect both macro-historical change and the microlevel community experiences of young people .
	manualset3
172983	4	410618	13	NULL	NULL	0	NULL	macro-historical change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of findings is that Black-White differences reflect both macro-historical change and the microlevel community experiences of young people .
	manualset3
172984	5	410618	13	NULL	NULL	0	NULL	microlevel community experiences	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of findings is that Black-White differences reflect both macro-historical change and the microlevel community experiences of young people .
	manualset3
172985	6	410618	13	NULL	NULL	0	NULL	young people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of findings is that Black-White differences reflect both macro-historical change and the microlevel community experiences of young people .
	manualset3
172986	1	410619	13	NULL	NULL	0	NULL	interpretation 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of the results , very dispersed at the present time , leads the authors two us two new clinical and histological indicators estimating the degree of severity of the prostatic cancer : the index of clinical severity based on the quality of survival and its duration from time T0 and the multifactorial index of histological severity based on the WHO classification , Gleason grade and NOR .
	manualset3
172987	2	410619	13	NULL	NULL	0	NULL	results 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of the results , very dispersed at the present time , leads the authors two us two new clinical and histological indicators estimating the degree of severity of the prostatic cancer : the index of clinical severity based on the quality of survival and its duration from time T0 and the multifactorial index of histological severity based on the WHO classification , Gleason grade and NOR .
	manualset3
172988	3	410619	13	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of the results , very dispersed at the present time , leads the authors two us two new clinical and histological indicators estimating the degree of severity of the prostatic cancer : the index of clinical severity based on the quality of survival and its duration from time T0 and the multifactorial index of histological severity based on the WHO classification , Gleason grade and NOR .
	manualset3
172989	4	410619	13	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of the results , very dispersed at the present time , leads the authors two us two new clinical and histological indicators estimating the degree of severity of the prostatic cancer : the index of clinical severity based on the quality of survival and its duration from time T0 and the multifactorial index of histological severity based on the WHO classification , Gleason grade and NOR .
	manualset3
172990	5	410619	13	NULL	NULL	0	NULL	two 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of the results , very dispersed at the present time , leads the authors two us two new clinical and histological indicators estimating the degree of severity of the prostatic cancer : the index of clinical severity based on the quality of survival and its duration from time T0 and the multifactorial index of histological severity based on the WHO classification , Gleason grade and NOR .
	manualset3
172991	6	410619	13	NULL	NULL	0	NULL	two 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of the results , very dispersed at the present time , leads the authors two us two new clinical and histological indicators estimating the degree of severity of the prostatic cancer : the index of clinical severity based on the quality of survival and its duration from time T0 and the multifactorial index of histological severity based on the WHO classification , Gleason grade and NOR .
	manualset3
172992	7	410619	13	NULL	NULL	0	NULL	clinical indicators 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of the results , very dispersed at the present time , leads the authors two us two new clinical and histological indicators estimating the degree of severity of the prostatic cancer : the index of clinical severity based on the quality of survival and its duration from time T0 and the multifactorial index of histological severity based on the WHO classification , Gleason grade and NOR .
	manualset3
172993	8	410619	13	NULL	NULL	0	NULL	degree of severity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of the results , very dispersed at the present time , leads the authors two us two new clinical and histological indicators estimating the degree of severity of the prostatic cancer : the index of clinical severity based on the quality of survival and its duration from time T0 and the multifactorial index of histological severity based on the WHO classification , Gleason grade and NOR .
	manualset3
172994	9	410619	13	NULL	NULL	0	NULL	prostatic cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of the results , very dispersed at the present time , leads the authors two us two new clinical and histological indicators estimating the degree of severity of the prostatic cancer : the index of clinical severity based on the quality of survival and its duration from time T0 and the multifactorial index of histological severity based on the WHO classification , Gleason grade and NOR .
	manualset3
172995	10	410619	13	NULL	NULL	0	NULL	index 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of the results , very dispersed at the present time , leads the authors two us two new clinical and histological indicators estimating the degree of severity of the prostatic cancer : the index of clinical severity based on the quality of survival and its duration from time T0 and the multifactorial index of histological severity based on the WHO classification , Gleason grade and NOR .
	manualset3
172996	11	410619	13	NULL	NULL	0	NULL	clinical severity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of the results , very dispersed at the present time , leads the authors two us two new clinical and histological indicators estimating the degree of severity of the prostatic cancer : the index of clinical severity based on the quality of survival and its duration from time T0 and the multifactorial index of histological severity based on the WHO classification , Gleason grade and NOR .
	manualset3
172997	12	410619	13	NULL	NULL	0	NULL	quality of survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of the results , very dispersed at the present time , leads the authors two us two new clinical and histological indicators estimating the degree of severity of the prostatic cancer : the index of clinical severity based on the quality of survival and its duration from time T0 and the multifactorial index of histological severity based on the WHO classification , Gleason grade and NOR .
	manualset3
172998	13	410619	13	NULL	NULL	0	NULL	duration 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of the results , very dispersed at the present time , leads the authors two us two new clinical and histological indicators estimating the degree of severity of the prostatic cancer : the index of clinical severity based on the quality of survival and its duration from time T0 and the multifactorial index of histological severity based on the WHO classification , Gleason grade and NOR .
	manualset3
172999	14	410619	13	NULL	NULL	0	NULL	time T0	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of the results , very dispersed at the present time , leads the authors two us two new clinical and histological indicators estimating the degree of severity of the prostatic cancer : the index of clinical severity based on the quality of survival and its duration from time T0 and the multifactorial index of histological severity based on the WHO classification , Gleason grade and NOR .
	manualset3
173000	15	410619	13	NULL	NULL	0	NULL	multifactorial index	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of the results , very dispersed at the present time , leads the authors two us two new clinical and histological indicators estimating the degree of severity of the prostatic cancer : the index of clinical severity based on the quality of survival and its duration from time T0 and the multifactorial index of histological severity based on the WHO classification , Gleason grade and NOR .
	manualset3
173001	16	410619	13	NULL	NULL	0	NULL	histological severity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of the results , very dispersed at the present time , leads the authors two us two new clinical and histological indicators estimating the degree of severity of the prostatic cancer : the index of clinical severity based on the quality of survival and its duration from time T0 and the multifactorial index of histological severity based on the WHO classification , Gleason grade and NOR .
	manualset3
173002	17	410619	13	NULL	NULL	0	NULL	WHO classification	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of the results , very dispersed at the present time , leads the authors two us two new clinical and histological indicators estimating the degree of severity of the prostatic cancer : the index of clinical severity based on the quality of survival and its duration from time T0 and the multifactorial index of histological severity based on the WHO classification , Gleason grade and NOR .
	manualset3
173003	18	410619	13	NULL	NULL	0	NULL	Gleason grade 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of the results , very dispersed at the present time , leads the authors two us two new clinical and histological indicators estimating the degree of severity of the prostatic cancer : the index of clinical severity based on the quality of survival and its duration from time T0 and the multifactorial index of histological severity based on the WHO classification , Gleason grade and NOR .
	manualset3
173004	19	410619	13	NULL	NULL	0	NULL	NOR 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of the results , very dispersed at the present time , leads the authors two us two new clinical and histological indicators estimating the degree of severity of the prostatic cancer : the index of clinical severity based on the quality of survival and its duration from time T0 and the multifactorial index of histological severity based on the WHO classification , Gleason grade and NOR .
	manualset3
178671	20	410619	13	NULL	NULL	0	NULL	histological indicators 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The interpretation of the results , very dispersed at the present time , leads the authors two us two new clinical and histological indicators estimating the degree of severity of the prostatic cancer : the index of clinical severity based on the quality of survival and its duration from time T0 and the multifactorial index of histological severity based on the WHO classification , Gleason grade and NOR .
	manualset3
173307	1	410620	13	NULL	NULL	0	NULL	interrelationship	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The interrelationship of membrane and protein structure in the functioning of the ( Na + = K + ) - activated ATPase .
	manualset3
173308	2	410620	13	NULL	NULL	0	NULL	membrane structure	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The interrelationship of membrane and protein structure in the functioning of the ( Na + = K + ) - activated ATPase .
	manualset3
173309	3	410620	13	NULL	NULL	0	NULL	protein structure 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The interrelationship of membrane and protein structure in the functioning of the ( Na + = K + ) - activated ATPase .
	manualset3
173310	4	410620	13	NULL	NULL	0	NULL	functioning	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The interrelationship of membrane and protein structure in the functioning of the ( Na + = K + ) - activated ATPase .
	manualset3
173311	5	410620	13	NULL	NULL	0	NULL	( Na + = K + ) - activated ATPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The interrelationship of membrane and protein structure in the functioning of the ( Na + = K + ) - activated ATPase .
	manualset3
173312	1	410621	13	NULL	NULL	NULL	NULL	interruption	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The interruption of TJ opening caused by Ca2 + , Cd2 + , or Mn2 + , and the stability they confer to the closed TJs , might result from the interaction of these ions with E-cadherin .
	manualset3
173313	2	410621	13	NULL	NULL	0	NULL	TJ opening	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The interruption of TJ opening caused by Ca2 + , Cd2 + , or Mn2 + , and the stability they confer to the closed TJs , might result from the interaction of these ions with E-cadherin .
	manualset3
173314	3	410621	13	NULL	NULL	0	NULL	Ca2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The interruption of TJ opening caused by Ca2 + , Cd2 + , or Mn2 + , and the stability they confer to the closed TJs , might result from the interaction of these ions with E-cadherin .
	manualset3
173315	4	410621	13	NULL	NULL	0	NULL	Cd2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The interruption of TJ opening caused by Ca2 + , Cd2 + , or Mn2 + , and the stability they confer to the closed TJs , might result from the interaction of these ions with E-cadherin .
	manualset3
173316	5	410621	13	NULL	NULL	0	NULL	Mn2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The interruption of TJ opening caused by Ca2 + , Cd2 + , or Mn2 + , and the stability they confer to the closed TJs , might result from the interaction of these ions with E-cadherin .
	manualset3
173317	6	410621	13	NULL	NULL	0	NULL	stability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The interruption of TJ opening caused by Ca2 + , Cd2 + , or Mn2 + , and the stability they confer to the closed TJs , might result from the interaction of these ions with E-cadherin .
	manualset3
173318	7	410621	13	NULL	NULL	0	NULL	TJs 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The interruption of TJ opening caused by Ca2 + , Cd2 + , or Mn2 + , and the stability they confer to the closed TJs , might result from the interaction of these ions with E-cadherin .
	manualset3
173319	8	410621	13	NULL	NULL	0	NULL	interaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The interruption of TJ opening caused by Ca2 + , Cd2 + , or Mn2 + , and the stability they confer to the closed TJs , might result from the interaction of these ions with E-cadherin .
	manualset3
173320	9	410621	13	NULL	NULL	0	NULL	ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The interruption of TJ opening caused by Ca2 + , Cd2 + , or Mn2 + , and the stability they confer to the closed TJs , might result from the interaction of these ions with E-cadherin .
	manualset3
173321	10	410621	13	NULL	NULL	0	NULL	E-cadherin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The interruption of TJ opening caused by Ca2 + , Cd2 + , or Mn2 + , and the stability they confer to the closed TJs , might result from the interaction of these ions with E-cadherin .
	manualset3
173322	1	410622	13	NULL	NULL	0	NULL	interspecific introgression analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The interspecific introgression analyses show that neither cytoplasm nor MHS genes are involved but X-Y interactions may be playing major role in hybrid male sterility between D. pseudoananassae and the other three species .
	manualset3
173323	2	410622	13	NULL	NULL	0	NULL	cytoplasm	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The interspecific introgression analyses show that neither cytoplasm nor MHS genes are involved but X-Y interactions may be playing major role in hybrid male sterility between D. pseudoananassae and the other three species .
	manualset3
173324	3	410622	13	NULL	NULL	0	NULL	MHS genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The interspecific introgression analyses show that neither cytoplasm nor MHS genes are involved but X-Y interactions may be playing major role in hybrid male sterility between D. pseudoananassae and the other three species .
	manualset3
173325	4	410622	13	NULL	NULL	0	NULL	 X-Y interactions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The interspecific introgression analyses show that neither cytoplasm nor MHS genes are involved but X-Y interactions may be playing major role in hybrid male sterility between D. pseudoananassae and the other three species .
	manualset3
173326	5	410622	13	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The interspecific introgression analyses show that neither cytoplasm nor MHS genes are involved but X-Y interactions may be playing major role in hybrid male sterility between D. pseudoananassae and the other three species .
	manualset3
173327	6	410622	13	NULL	NULL	0	NULL	male sterility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The interspecific introgression analyses show that neither cytoplasm nor MHS genes are involved but X-Y interactions may be playing major role in hybrid male sterility between D. pseudoananassae and the other three species .
	manualset3
173328	7	410622	13	NULL	NULL	0	NULL	D. pseudoananassae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The interspecific introgression analyses show that neither cytoplasm nor MHS genes are involved but X-Y interactions may be playing major role in hybrid male sterility between D. pseudoananassae and the other three species .
	manualset3
173329	8	410622	13	NULL	NULL	0	NULL	three species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The interspecific introgression analyses show that neither cytoplasm nor MHS genes are involved but X-Y interactions may be playing major role in hybrid male sterility between D. pseudoananassae and the other three species .
	manualset3
173330	1	410623	13	NULL	NULL	0	NULL	interval	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The interval between subsequent collections had a large effect on sperm concentration .
	manualset3
173331	2	410623	13	NULL	NULL	0	NULL	collections	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The interval between subsequent collections had a large effect on sperm concentration .
	manualset3
173332	3	410623	13	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The interval between subsequent collections had a large effect on sperm concentration .
	manualset3
173333	4	410623	13	NULL	NULL	0	NULL	sperm concentration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The interval between subsequent collections had a large effect on sperm concentration .
	manualset3
173339	1	410624	13	NULL	NULL	0	NULL	intervention group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The intervention group had a 20 % reduction in ED visits , which was significant compared with the control group ( p = 0.017 ) ; both groups had significant reductions in hospitalizations .
	manualset3
173342	2	410624	13	NULL	NULL	0	NULL	20 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The intervention group had a 20 % reduction in ED visits , which was significant compared with the control group ( p = 0.017 ) ; both groups had significant reductions in hospitalizations .
	manualset3
173343	3	410624	13	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The intervention group had a 20 % reduction in ED visits , which was significant compared with the control group ( p = 0.017 ) ; both groups had significant reductions in hospitalizations .
	manualset3
173345	4	410624	13	NULL	NULL	0	NULL	ED visits	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The intervention group had a 20 % reduction in ED visits , which was significant compared with the control group ( p = 0.017 ) ; both groups had significant reductions in hospitalizations .
	manualset3
173355	5	410624	13	NULL	NULL	0	NULL	control group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The intervention group had a 20 % reduction in ED visits , which was significant compared with the control group ( p = 0.017 ) ; both groups had significant reductions in hospitalizations .
	manualset3
173356	6	410624	13	NULL	NULL	0	NULL	p = 0.017	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The intervention group had a 20 % reduction in ED visits , which was significant compared with the control group ( p = 0.017 ) ; both groups had significant reductions in hospitalizations .
	manualset3
173357	7	410624	13	NULL	NULL	0	NULL	groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The intervention group had a 20 % reduction in ED visits , which was significant compared with the control group ( p = 0.017 ) ; both groups had significant reductions in hospitalizations .
	manualset3
173358	8	410624	13	NULL	NULL	0	NULL	reductions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The intervention group had a 20 % reduction in ED visits , which was significant compared with the control group ( p = 0.017 ) ; both groups had significant reductions in hospitalizations .
	manualset3
173360	9	410624	13	NULL	NULL	0	NULL	hospitalizations 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The intervention group had a 20 % reduction in ED visits , which was significant compared with the control group ( p = 0.017 ) ; both groups had significant reductions in hospitalizations .
	manualset3
173364	1	410625	13	NULL	NULL	0	NULL	interventions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The interventions , which are conducted at work sites , schools , health care centers and in community settings rely on partnerships created among professionals in areas of education and health , business officials and personnel , and community members , to deliver the programs in each of these settings and populations .
	manualset3
173365	2	410625	13	NULL	NULL	NULL	NULL	work sites	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The interventions , which are conducted at work sites , schools , health care centers and in community settings rely on partnerships created among professionals in areas of education and health , business officials and personnel , and community members , to deliver the programs in each of these settings and populations .
	manualset3
173366	3	410625	13	NULL	NULL	0	NULL	schools	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The interventions , which are conducted at work sites , schools , health care centers and in community settings rely on partnerships created among professionals in areas of education and health , business officials and personnel , and community members , to deliver the programs in each of these settings and populations .
	manualset3
173367	4	410625	13	NULL	NULL	0	NULL	health care centers 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The interventions , which are conducted at work sites , schools , health care centers and in community settings rely on partnerships created among professionals in areas of education and health , business officials and personnel , and community members , to deliver the programs in each of these settings and populations .
	manualset3
173368	5	410625	13	NULL	NULL	0	NULL	community settings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The interventions , which are conducted at work sites , schools , health care centers and in community settings rely on partnerships created among professionals in areas of education and health , business officials and personnel , and community members , to deliver the programs in each of these settings and populations .
	manualset3
173369	6	410625	13	NULL	NULL	0	NULL	partnerships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The interventions , which are conducted at work sites , schools , health care centers and in community settings rely on partnerships created among professionals in areas of education and health , business officials and personnel , and community members , to deliver the programs in each of these settings and populations .
	manualset3
173370	7	410625	13	NULL	NULL	0	NULL	professionals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The interventions , which are conducted at work sites , schools , health care centers and in community settings rely on partnerships created among professionals in areas of education and health , business officials and personnel , and community members , to deliver the programs in each of these settings and populations .
	manualset3
173371	8	410625	13	NULL	NULL	0	NULL	areas of education	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The interventions , which are conducted at work sites , schools , health care centers and in community settings rely on partnerships created among professionals in areas of education and health , business officials and personnel , and community members , to deliver the programs in each of these settings and populations .
	manualset3
173372	9	410625	13	NULL	NULL	0	NULL	areas of health	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The interventions , which are conducted at work sites , schools , health care centers and in community settings rely on partnerships created among professionals in areas of education and health , business officials and personnel , and community members , to deliver the programs in each of these settings and populations .
	manualset3
173373	10	410625	13	NULL	NULL	0	NULL	business officials	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The interventions , which are conducted at work sites , schools , health care centers and in community settings rely on partnerships created among professionals in areas of education and health , business officials and personnel , and community members , to deliver the programs in each of these settings and populations .
	manualset3
173374	11	410625	13	NULL	NULL	0	NULL	personnel 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The interventions , which are conducted at work sites , schools , health care centers and in community settings rely on partnerships created among professionals in areas of education and health , business officials and personnel , and community members , to deliver the programs in each of these settings and populations .
	manualset3
173375	12	410625	13	NULL	NULL	0	NULL	community members 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The interventions , which are conducted at work sites , schools , health care centers and in community settings rely on partnerships created among professionals in areas of education and health , business officials and personnel , and community members , to deliver the programs in each of these settings and populations .
	manualset3
173376	13	410625	13	NULL	NULL	0	NULL	programs 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The interventions , which are conducted at work sites , schools , health care centers and in community settings rely on partnerships created among professionals in areas of education and health , business officials and personnel , and community members , to deliver the programs in each of these settings and populations .
	manualset3
173377	14	410625	13	NULL	NULL	0	NULL	settings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The interventions , which are conducted at work sites , schools , health care centers and in community settings rely on partnerships created among professionals in areas of education and health , business officials and personnel , and community members , to deliver the programs in each of these settings and populations .
	manualset3
173378	15	410625	13	NULL	NULL	0	NULL	 populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The interventions , which are conducted at work sites , schools , health care centers and in community settings rely on partnerships created among professionals in areas of education and health , business officials and personnel , and community members , to deliver the programs in each of these settings and populations .
	manualset3
173379	1	410626	13	NULL	NULL	0	NULL	interviews	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The interviews were analyzed with regard to coherence of speech , coping with emotional problems , reflectivity , child representation of both parents , and verbal and nonverbal expression of feelings .
	manualset3
173380	2	410626	13	NULL	NULL	0	NULL	regard	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The interviews were analyzed with regard to coherence of speech , coping with emotional problems , reflectivity , child representation of both parents , and verbal and nonverbal expression of feelings .
	manualset3
173381	3	410626	13	NULL	NULL	0	NULL	coherence of speech 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The interviews were analyzed with regard to coherence of speech , coping with emotional problems , reflectivity , child representation of both parents , and verbal and nonverbal expression of feelings .
	manualset3
173382	4	410626	13	NULL	NULL	NULL	NULL	emotional problems	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The interviews were analyzed with regard to coherence of speech , coping with emotional problems , reflectivity , child representation of both parents , and verbal and nonverbal expression of feelings .
	manualset3
173383	5	410626	13	NULL	NULL	NULL	NULL	reflectivity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The interviews were analyzed with regard to coherence of speech , coping with emotional problems , reflectivity , child representation of both parents , and verbal and nonverbal expression of feelings .
	manualset3
173384	6	410626	13	NULL	NULL	0	NULL	child representation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The interviews were analyzed with regard to coherence of speech , coping with emotional problems , reflectivity , child representation of both parents , and verbal and nonverbal expression of feelings .
	manualset3
173385	7	410626	13	NULL	NULL	0	NULL	parents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The interviews were analyzed with regard to coherence of speech , coping with emotional problems , reflectivity , child representation of both parents , and verbal and nonverbal expression of feelings .
	manualset3
173386	8	410626	13	NULL	NULL	0	NULL	verbal expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The interviews were analyzed with regard to coherence of speech , coping with emotional problems , reflectivity , child representation of both parents , and verbal and nonverbal expression of feelings .
	manualset3
173387	9	410626	13	NULL	NULL	0	NULL	nonverbal expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The interviews were analyzed with regard to coherence of speech , coping with emotional problems , reflectivity , child representation of both parents , and verbal and nonverbal expression of feelings .
	manualset3
173388	10	410626	13	NULL	NULL	0	NULL	feelings	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The interviews were analyzed with regard to coherence of speech , coping with emotional problems , reflectivity , child representation of both parents , and verbal and nonverbal expression of feelings .
	manualset3
173389	1	410627	13	NULL	NULL	0	NULL	intracellular distribution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The intracellular distribution of vinculin and alpha 2 integrin in epithelial cells and chondrocytes .
	manualset3
173390	2	410627	13	NULL	NULL	0	NULL	vinculin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The intracellular distribution of vinculin and alpha 2 integrin in epithelial cells and chondrocytes .
	manualset3
173391	3	410627	13	NULL	NULL	0	NULL	alpha 2 integrin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The intracellular distribution of vinculin and alpha 2 integrin in epithelial cells and chondrocytes .
	manualset3
173392	4	410627	13	NULL	NULL	0	NULL	epithelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The intracellular distribution of vinculin and alpha 2 integrin in epithelial cells and chondrocytes .
	manualset3
173393	5	410627	13	NULL	NULL	0	NULL	chondrocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The intracellular distribution of vinculin and alpha 2 integrin in epithelial cells and chondrocytes .
	manualset3
173394	1	410628	13	NULL	NULL	0	NULL	intracellular half-lives	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The intracellular half-lives of L-dTTP , L-dCTP , and L-dUTP were at least 15 h , with intracellular concentrations of each metabolite remaining above their respective 50 % inhibitory concentrations for the woodchuck hepatitis virus DNA polymerase for as long as 24 h after removal of the drug from cell cultures .
	manualset3
173395	2	410628	13	NULL	NULL	0	NULL	L-dTTP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The intracellular half-lives of L-dTTP , L-dCTP , and L-dUTP were at least 15 h , with intracellular concentrations of each metabolite remaining above their respective 50 % inhibitory concentrations for the woodchuck hepatitis virus DNA polymerase for as long as 24 h after removal of the drug from cell cultures .
	manualset3
173396	3	410628	13	NULL	NULL	0	NULL	L-dCTP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The intracellular half-lives of L-dTTP , L-dCTP , and L-dUTP were at least 15 h , with intracellular concentrations of each metabolite remaining above their respective 50 % inhibitory concentrations for the woodchuck hepatitis virus DNA polymerase for as long as 24 h after removal of the drug from cell cultures .
	manualset3
173397	4	410628	13	NULL	NULL	0	NULL	L-dUTP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The intracellular half-lives of L-dTTP , L-dCTP , and L-dUTP were at least 15 h , with intracellular concentrations of each metabolite remaining above their respective 50 % inhibitory concentrations for the woodchuck hepatitis virus DNA polymerase for as long as 24 h after removal of the drug from cell cultures .
	manualset3
173398	5	410628	13	NULL	NULL	0	NULL	15 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The intracellular half-lives of L-dTTP , L-dCTP , and L-dUTP were at least 15 h , with intracellular concentrations of each metabolite remaining above their respective 50 % inhibitory concentrations for the woodchuck hepatitis virus DNA polymerase for as long as 24 h after removal of the drug from cell cultures .
	manualset3
173399	6	410628	13	NULL	NULL	0	NULL	intracellular concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The intracellular half-lives of L-dTTP , L-dCTP , and L-dUTP were at least 15 h , with intracellular concentrations of each metabolite remaining above their respective 50 % inhibitory concentrations for the woodchuck hepatitis virus DNA polymerase for as long as 24 h after removal of the drug from cell cultures .
	manualset3
173400	7	410628	13	NULL	NULL	0	NULL	metabolite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The intracellular half-lives of L-dTTP , L-dCTP , and L-dUTP were at least 15 h , with intracellular concentrations of each metabolite remaining above their respective 50 % inhibitory concentrations for the woodchuck hepatitis virus DNA polymerase for as long as 24 h after removal of the drug from cell cultures .
	manualset3
173401	8	410628	13	NULL	NULL	0	NULL	50 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The intracellular half-lives of L-dTTP , L-dCTP , and L-dUTP were at least 15 h , with intracellular concentrations of each metabolite remaining above their respective 50 % inhibitory concentrations for the woodchuck hepatitis virus DNA polymerase for as long as 24 h after removal of the drug from cell cultures .
	manualset3
173402	9	410628	13	NULL	NULL	0	NULL	concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The intracellular half-lives of L-dTTP , L-dCTP , and L-dUTP were at least 15 h , with intracellular concentrations of each metabolite remaining above their respective 50 % inhibitory concentrations for the woodchuck hepatitis virus DNA polymerase for as long as 24 h after removal of the drug from cell cultures .
	manualset3
173403	10	410628	13	NULL	NULL	0	NULL	woodchuck hepatitis virus DNA polymerase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The intracellular half-lives of L-dTTP , L-dCTP , and L-dUTP were at least 15 h , with intracellular concentrations of each metabolite remaining above their respective 50 % inhibitory concentrations for the woodchuck hepatitis virus DNA polymerase for as long as 24 h after removal of the drug from cell cultures .
	manualset3
173404	11	410628	13	NULL	NULL	0	NULL	24 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The intracellular half-lives of L-dTTP , L-dCTP , and L-dUTP were at least 15 h , with intracellular concentrations of each metabolite remaining above their respective 50 % inhibitory concentrations for the woodchuck hepatitis virus DNA polymerase for as long as 24 h after removal of the drug from cell cultures .
	manualset3
173405	12	410628	13	NULL	NULL	0	NULL	removal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The intracellular half-lives of L-dTTP , L-dCTP , and L-dUTP were at least 15 h , with intracellular concentrations of each metabolite remaining above their respective 50 % inhibitory concentrations for the woodchuck hepatitis virus DNA polymerase for as long as 24 h after removal of the drug from cell cultures .
	manualset3
173406	13	410628	13	NULL	NULL	0	NULL	drug 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The intracellular half-lives of L-dTTP , L-dCTP , and L-dUTP were at least 15 h , with intracellular concentrations of each metabolite remaining above their respective 50 % inhibitory concentrations for the woodchuck hepatitis virus DNA polymerase for as long as 24 h after removal of the drug from cell cultures .
	manualset3
173407	14	410628	13	NULL	NULL	0	NULL	cell cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The intracellular half-lives of L-dTTP , L-dCTP , and L-dUTP were at least 15 h , with intracellular concentrations of each metabolite remaining above their respective 50 % inhibitory concentrations for the woodchuck hepatitis virus DNA polymerase for as long as 24 h after removal of the drug from cell cultures .
	manualset3
173413	1	410629	13	NULL	NULL	0	NULL	intracellular location 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The intracellular location of GLUT4 in the basal state and the pathway by which it reaches the cell surface upon insulin stimulation are unclear .
	manualset3
173414	2	410629	13	NULL	NULL	0	NULL	GLUT4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The intracellular location of GLUT4 in the basal state and the pathway by which it reaches the cell surface upon insulin stimulation are unclear .
	manualset3
173415	3	410629	13	NULL	NULL	0	NULL	basal state 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The intracellular location of GLUT4 in the basal state and the pathway by which it reaches the cell surface upon insulin stimulation are unclear .
	manualset3
173624	4	410629	13	NULL	NULL	0	NULL	pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The intracellular location of GLUT4 in the basal state and the pathway by which it reaches the cell surface upon insulin stimulation are unclear .
	manualset3
173625	5	410629	13	NULL	NULL	0	NULL	cell surface	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The intracellular location of GLUT4 in the basal state and the pathway by which it reaches the cell surface upon insulin stimulation are unclear .
	manualset3
173626	6	410629	13	NULL	NULL	0	NULL	insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The intracellular location of GLUT4 in the basal state and the pathway by which it reaches the cell surface upon insulin stimulation are unclear .
	manualset3
173627	7	410629	13	NULL	NULL	0	NULL	stimulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The intracellular location of GLUT4 in the basal state and the pathway by which it reaches the cell surface upon insulin stimulation are unclear .
	manualset3
173628	1	410630	13	NULL	NULL	NULL	NULL	intranasal quercetin liposomes 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The intranasal quercetin liposomes are effective in the delivery of quercetin to the central nervous system .
	manualset3
173629	2	410630	13	NULL	NULL	0	NULL	delivery	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The intranasal quercetin liposomes are effective in the delivery of quercetin to the central nervous system .
	manualset3
173630	3	410630	13	NULL	NULL	0	NULL	quercetin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The intranasal quercetin liposomes are effective in the delivery of quercetin to the central nervous system .
	manualset3
173631	4	410630	13	NULL	NULL	0	NULL	central nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The intranasal quercetin liposomes are effective in the delivery of quercetin to the central nervous system .
	manualset3
173632	1	410631	13	NULL	NULL	0	NULL	intranasal trigeminal system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The intranasal trigeminal system is a third chemical sense in addition to olfaction and gustation .
	manualset3
173633	2	410631	13	NULL	NULL	0	NULL	third chemical sense 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The intranasal trigeminal system is a third chemical sense in addition to olfaction and gustation .
	manualset3
173634	3	410631	13	NULL	NULL	0	NULL	olfaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The intranasal trigeminal system is a third chemical sense in addition to olfaction and gustation .
	manualset3
173635	4	410631	13	NULL	NULL	0	NULL	gustation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The intranasal trigeminal system is a third chemical sense in addition to olfaction and gustation .
	manualset3
173636	1	410632	13	NULL	NULL	0	NULL	T cell activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The intrinsic T cell activity of Igha mice against IgG2ab ( IgG2a from the Ighb haplotype ) can be subjected to profound specific tolerance .
	manualset3
173637	2	410632	13	NULL	NULL	0	NULL	Igha mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The intrinsic T cell activity of Igha mice against IgG2ab ( IgG2a from the Ighb haplotype ) can be subjected to profound specific tolerance .
	manualset3
173638	3	410632	13	NULL	NULL	0	NULL	IgG2ab 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The intrinsic T cell activity of Igha mice against IgG2ab ( IgG2a from the Ighb haplotype ) can be subjected to profound specific tolerance .
	manualset3
173639	4	410632	13	NULL	NULL	0	NULL	IgG2a	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The intrinsic T cell activity of Igha mice against IgG2ab ( IgG2a from the Ighb haplotype ) can be subjected to profound specific tolerance .
	manualset3
173640	5	410632	13	NULL	NULL	0	NULL	Ighb haplotype 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The intrinsic T cell activity of Igha mice against IgG2ab ( IgG2a from the Ighb haplotype ) can be subjected to profound specific tolerance .
	manualset3
173641	6	410632	13	NULL	NULL	0	NULL	tolerance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The intrinsic T cell activity of Igha mice against IgG2ab ( IgG2a from the Ighb haplotype ) can be subjected to profound specific tolerance .
	manualset3
173674	1	410633	13	NULL	NULL	0	NULL	 introduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The introduction discusses current theoretical concepts and basic functional approaches in vertebrate morphology .
	manualset3
173675	2	410633	13	NULL	NULL	0	NULL	theoretical concepts	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The introduction discusses current theoretical concepts and basic functional approaches in vertebrate morphology .
	manualset3
173676	3	410633	13	NULL	NULL	0	NULL	functional approaches	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The introduction discusses current theoretical concepts and basic functional approaches in vertebrate morphology .
	manualset3
173677	4	410633	13	NULL	NULL	0	NULL	vertebrate morphology	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The introduction discusses current theoretical concepts and basic functional approaches in vertebrate morphology .
	manualset3
173678	1	410634	13	NULL	NULL	0	NULL	total	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 279 cases and 307 controls were compared for sociodemographic characteristics , cigarette smoking , sexual reproductive and surgical histories and for the conditions under which conception occurred .
	manualset3
173679	2	410634	13	NULL	NULL	0	NULL	279 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 279 cases and 307 controls were compared for sociodemographic characteristics , cigarette smoking , sexual reproductive and surgical histories and for the conditions under which conception occurred .
	manualset3
173681	3	410634	13	NULL	NULL	0	NULL	307 controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 279 cases and 307 controls were compared for sociodemographic characteristics , cigarette smoking , sexual reproductive and surgical histories and for the conditions under which conception occurred .
	manualset3
173684	4	410634	13	NULL	NULL	0	NULL	sociodemographic characteristics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 279 cases and 307 controls were compared for sociodemographic characteristics , cigarette smoking , sexual reproductive and surgical histories and for the conditions under which conception occurred .
	manualset3
173685	5	410634	13	NULL	NULL	0	NULL	cigarette 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 279 cases and 307 controls were compared for sociodemographic characteristics , cigarette smoking , sexual reproductive and surgical histories and for the conditions under which conception occurred .
	manualset3
173686	6	410634	13	NULL	NULL	0	NULL	sexual reproductive histories	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 279 cases and 307 controls were compared for sociodemographic characteristics , cigarette smoking , sexual reproductive and surgical histories and for the conditions under which conception occurred .
	manualset3
173687	7	410634	13	NULL	NULL	0	NULL	surgical histories	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 279 cases and 307 controls were compared for sociodemographic characteristics , cigarette smoking , sexual reproductive and surgical histories and for the conditions under which conception occurred .
	manualset3
173688	8	410634	13	NULL	NULL	0	NULL	conditions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 279 cases and 307 controls were compared for sociodemographic characteristics , cigarette smoking , sexual reproductive and surgical histories and for the conditions under which conception occurred .
	manualset3
173689	9	410634	13	NULL	NULL	0	NULL	conception	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 279 cases and 307 controls were compared for sociodemographic characteristics , cigarette smoking , sexual reproductive and surgical histories and for the conditions under which conception occurred .
	manualset3
173691	1	410635	13	NULL	NULL	0	NULL	introduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The introduction of air bubbles into the systemic circulation can result in significant morbidity .
	manualset3
173692	2	410635	13	NULL	NULL	0	NULL	air bubbles	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The introduction of air bubbles into the systemic circulation can result in significant morbidity .
	manualset3
173693	3	410635	13	NULL	NULL	0	NULL	systemic circulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The introduction of air bubbles into the systemic circulation can result in significant morbidity .
	manualset3
173694	4	410635	13	NULL	NULL	0	NULL	morbidity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The introduction of air bubbles into the systemic circulation can result in significant morbidity .
	manualset3
173823	1	410636	13	NULL	NULL	0	NULL	introduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The introduction of negatively charged and hydrophobic amino acids resulted in a decrease in secretion efficiency and impaired the SP-APL interaction , whereas His and Tyr had no significant effect .
	manualset3
173824	2	410636	13	NULL	NULL	0	NULL	negatively charged amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The introduction of negatively charged and hydrophobic amino acids resulted in a decrease in secretion efficiency and impaired the SP-APL interaction , whereas His and Tyr had no significant effect .
	manualset3
173825	3	410636	13	NULL	NULL	0	NULL	 hydrophobic amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The introduction of negatively charged and hydrophobic amino acids resulted in a decrease in secretion efficiency and impaired the SP-APL interaction , whereas His and Tyr had no significant effect .
	manualset3
173826	4	410636	13	NULL	NULL	0	NULL	decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The introduction of negatively charged and hydrophobic amino acids resulted in a decrease in secretion efficiency and impaired the SP-APL interaction , whereas His and Tyr had no significant effect .
	manualset3
173827	5	410636	13	NULL	NULL	0	NULL	secretion efficiency 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The introduction of negatively charged and hydrophobic amino acids resulted in a decrease in secretion efficiency and impaired the SP-APL interaction , whereas His and Tyr had no significant effect .
	manualset3
173828	6	410636	13	NULL	NULL	0	NULL	SP-APL interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The introduction of negatively charged and hydrophobic amino acids resulted in a decrease in secretion efficiency and impaired the SP-APL interaction , whereas His and Tyr had no significant effect .
	manualset3
173829	7	410636	13	NULL	NULL	0	NULL	His	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The introduction of negatively charged and hydrophobic amino acids resulted in a decrease in secretion efficiency and impaired the SP-APL interaction , whereas His and Tyr had no significant effect .
	manualset3
173831	8	410636	13	NULL	NULL	0	NULL	Tyr 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The introduction of negatively charged and hydrophobic amino acids resulted in a decrease in secretion efficiency and impaired the SP-APL interaction , whereas His and Tyr had no significant effect .
	manualset3
173832	9	410636	13	NULL	NULL	0	NULL	effect 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The introduction of negatively charged and hydrophobic amino acids resulted in a decrease in secretion efficiency and impaired the SP-APL interaction , whereas His and Tyr had no significant effect .
	manualset3
173838	1	410637	13	NULL	NULL	0	NULL	introns 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The introns of tubulin genes , many of them clustered in the first quarter of the tubulin coding region , do not appear to correspond to any particular structural or functional regions .
	manualset3
173839	2	410637	13	NULL	NULL	0	NULL	tubulin genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The introns of tubulin genes , many of them clustered in the first quarter of the tubulin coding region , do not appear to correspond to any particular structural or functional regions .
	manualset3
173842	3	410637	13	NULL	NULL	0	NULL	first quarter	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The introns of tubulin genes , many of them clustered in the first quarter of the tubulin coding region , do not appear to correspond to any particular structural or functional regions .
	manualset3
173843	4	410637	13	NULL	NULL	0	NULL	tubulin coding region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The introns of tubulin genes , many of them clustered in the first quarter of the tubulin coding region , do not appear to correspond to any particular structural or functional regions .
	manualset3
173844	5	410637	13	NULL	NULL	0	NULL	structural regions	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The introns of tubulin genes , many of them clustered in the first quarter of the tubulin coding region , do not appear to correspond to any particular structural or functional regions .
	manualset3
173845	6	410637	13	NULL	NULL	0	NULL	functional regions 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The introns of tubulin genes , many of them clustered in the first quarter of the tubulin coding region , do not appear to correspond to any particular structural or functional regions .
	manualset3
173846	1	410638	13	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The inverse association between PA and BPH risk may be due to favorable hormonal correlates of PA , but residual confounding by socioeconomic covariates can not be excluded .
	manualset3
173847	2	410638	13	NULL	NULL	0	NULL	PA	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The inverse association between PA and BPH risk may be due to favorable hormonal correlates of PA , but residual confounding by socioeconomic covariates can not be excluded .
	manualset3
173848	3	410638	13	NULL	NULL	0	NULL	BPH risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The inverse association between PA and BPH risk may be due to favorable hormonal correlates of PA , but residual confounding by socioeconomic covariates can not be excluded .
	manualset3
173849	4	410638	13	NULL	NULL	0	NULL	hormonal correlates	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The inverse association between PA and BPH risk may be due to favorable hormonal correlates of PA , but residual confounding by socioeconomic covariates can not be excluded .
	manualset3
173850	5	410638	13	NULL	NULL	0	NULL	PA 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The inverse association between PA and BPH risk may be due to favorable hormonal correlates of PA , but residual confounding by socioeconomic covariates can not be excluded .
	manualset3
173851	6	410638	13	NULL	NULL	NULL	NULL	socioeconomic covariates	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The inverse association between PA and BPH risk may be due to favorable hormonal correlates of PA , but residual confounding by socioeconomic covariates can not be excluded .
	manualset3
173857	1	410639	13	NULL	NULL	0	NULL	ratio	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The inverted ratio was due to a deficiency in T-helper cells .
	manualset3
173858	2	410639	13	NULL	NULL	0	NULL	deficiency 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The inverted ratio was due to a deficiency in T-helper cells .
	manualset3
173859	3	410639	13	NULL	NULL	0	NULL	T-helper cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The inverted ratio was due to a deficiency in T-helper cells .
	manualset3
173860	1	410640	13	NULL	NULL	0	NULL	investigation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The investigation on calcium ( II ) oxalate is carried out in order to study its solubility in different ionic media .
	manualset3
173861	2	410640	13	NULL	NULL	0	NULL	calcium ( II ) oxalate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The investigation on calcium ( II ) oxalate is carried out in order to study its solubility in different ionic media .
	manualset3
173862	3	410640	13	NULL	NULL	0	NULL	solubility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The investigation on calcium ( II ) oxalate is carried out in order to study its solubility in different ionic media .
	manualset3
173863	4	410640	13	NULL	NULL	0	NULL	ionic media	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The investigation on calcium ( II ) oxalate is carried out in order to study its solubility in different ionic media .
	manualset3
173864	1	410641	13	NULL	NULL	NULL	NULL	investigations	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The investigations were based on small-angle X-ray scattering ( SAXS ) and rheometry techniques .
	manualset3
173865	2	410641	13	NULL	NULL	0	NULL	small-angle X-ray scattering ( SAXS ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The investigations were based on small-angle X-ray scattering ( SAXS ) and rheometry techniques .
	manualset3
173866	3	410641	13	NULL	NULL	0	NULL	rheometry techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The investigations were based on small-angle X-ray scattering ( SAXS ) and rheometry techniques .
	manualset3
173867	1	410642	13	NULL	NULL	0	NULL	involvement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The involvement of G proteins and regulators of receptor-G protein coupling in the pathophysiology , diagnosis and treatment of mood disorders .
	manualset3
173868	2	410642	13	NULL	NULL	0	NULL	G proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The involvement of G proteins and regulators of receptor-G protein coupling in the pathophysiology , diagnosis and treatment of mood disorders .
	manualset3
173869	3	410642	13	NULL	NULL	0	NULL	regulators	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The involvement of G proteins and regulators of receptor-G protein coupling in the pathophysiology , diagnosis and treatment of mood disorders .
	manualset3
173870	4	410642	13	NULL	NULL	0	NULL	receptor-G protein coupling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The involvement of G proteins and regulators of receptor-G protein coupling in the pathophysiology , diagnosis and treatment of mood disorders .
	manualset3
173871	5	410642	13	NULL	NULL	0	NULL	pathophysiology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The involvement of G proteins and regulators of receptor-G protein coupling in the pathophysiology , diagnosis and treatment of mood disorders .
	manualset3
173872	6	410642	13	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The involvement of G proteins and regulators of receptor-G protein coupling in the pathophysiology , diagnosis and treatment of mood disorders .
	manualset3
173873	7	410642	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The involvement of G proteins and regulators of receptor-G protein coupling in the pathophysiology , diagnosis and treatment of mood disorders .
	manualset3
173874	8	410642	13	NULL	NULL	NULL	NULL	mood disorders	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The involvement of G proteins and regulators of receptor-G protein coupling in the pathophysiology , diagnosis and treatment of mood disorders .
	manualset3
173875	1	410643	13	NULL	NULL	0	NULL	involvement 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The involvement of HLA antigens is detailed .
	manualset3
173876	2	410643	13	NULL	NULL	0	NULL	HLA antigens 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The involvement of HLA antigens is detailed .
	manualset3
173877	1	410644	13	NULL	NULL	0	NULL	CD34 + cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolated CD34 + cells were immunophenotyped using CD34-allophycocyanin , CD38-fluorescein isothiocyanate , and Thy-1-phycoerythrin .
	manualset3
173878	2	410644	13	NULL	NULL	0	NULL	CD34-allophycocyanin	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolated CD34 + cells were immunophenotyped using CD34-allophycocyanin , CD38-fluorescein isothiocyanate , and Thy-1-phycoerythrin .
	manualset3
173879	3	410644	13	NULL	NULL	0	NULL	CD38-fluorescein isothiocyanate	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolated CD34 + cells were immunophenotyped using CD34-allophycocyanin , CD38-fluorescein isothiocyanate , and Thy-1-phycoerythrin .
	manualset3
173880	4	410644	13	NULL	NULL	0	NULL	Thy-1-phycoerythrin	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolated CD34 + cells were immunophenotyped using CD34-allophycocyanin , CD38-fluorescein isothiocyanate , and Thy-1-phycoerythrin .
	manualset3
173881	1	410645	13	NULL	NULL	0	NULL	isolation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolation and characterization of a human functional GRP78 gene and a processed pseudogene are described .
	manualset3
173882	2	410645	13	NULL	NULL	0	NULL	characterization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolation and characterization of a human functional GRP78 gene and a processed pseudogene are described .
	manualset3
173883	3	410645	13	NULL	NULL	0	NULL	human functional GRP78 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolation and characterization of a human functional GRP78 gene and a processed pseudogene are described .
	manualset3
173884	4	410645	13	NULL	NULL	0	NULL	pseudogene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolation and characterization of a human functional GRP78 gene and a processed pseudogene are described .
	manualset3
173885	1	410646	13	NULL	NULL	0	NULL	isolation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolation and identification of Trypanosoma cruzi from raccoons in Maryland .
	manualset3
173886	2	410646	13	NULL	NULL	0	NULL	identification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolation and identification of Trypanosoma cruzi from raccoons in Maryland .
	manualset3
173887	3	410646	13	NULL	NULL	0	NULL	Trypanosoma cruzi	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolation and identification of Trypanosoma cruzi from raccoons in Maryland .
	manualset3
173888	4	410646	13	NULL	NULL	0	NULL	raccoons	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolation and identification of Trypanosoma cruzi from raccoons in Maryland .
	manualset3
173889	5	410646	13	NULL	NULL	0	NULL	Maryland	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolation and identification of Trypanosoma cruzi from raccoons in Maryland .
	manualset3
173890	1	410647	13	NULL	NULL	0	NULL	Clinical aspects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical aspects and therapy of the advanced stages of malignant melanoma ) .
	manualset3
173891	2	410647	13	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical aspects and therapy of the advanced stages of malignant melanoma ) .
	manualset3
173892	3	410647	13	NULL	NULL	0	NULL	advanced stages	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical aspects and therapy of the advanced stages of malignant melanoma ) .
	manualset3
173893	4	410647	13	NULL	NULL	0	NULL	malignant melanoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical aspects and therapy of the advanced stages of malignant melanoma ) .
	manualset3
173894	1	410648	13	NULL	NULL	0	NULL	isolation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolation and sequencing of pMC1 integration sites from these bacteria showed that in lactobacilli , pMC1 integrated into the conserved tRNA ( Ser ) gene .
	manualset3
173895	2	410648	13	NULL	NULL	0	NULL	pMC1 integration sites	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolation and sequencing of pMC1 integration sites from these bacteria showed that in lactobacilli , pMC1 integrated into the conserved tRNA ( Ser ) gene .
	manualset3
173896	3	410648	13	NULL	NULL	0	NULL	bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolation and sequencing of pMC1 integration sites from these bacteria showed that in lactobacilli , pMC1 integrated into the conserved tRNA ( Ser ) gene .
	manualset3
173897	4	410648	13	NULL	NULL	0	NULL	lactobacilli 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolation and sequencing of pMC1 integration sites from these bacteria showed that in lactobacilli , pMC1 integrated into the conserved tRNA ( Ser ) gene .
	manualset3
173898	5	410648	13	NULL	NULL	0	NULL	pMC1	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolation and sequencing of pMC1 integration sites from these bacteria showed that in lactobacilli , pMC1 integrated into the conserved tRNA ( Ser ) gene .
	manualset3
173899	6	410648	13	NULL	NULL	0	NULL	tRNA ( Ser ) gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolation and sequencing of pMC1 integration sites from these bacteria showed that in lactobacilli , pMC1 integrated into the conserved tRNA ( Ser ) gene .
	manualset3
173900	1	410649	13	NULL	NULL	0	NULL	isolation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolation of individual proteins from whey would allow production of more consistent and reliable products by the food industry and possibly would also increase their use in the pharmaceutical industry .
	manualset3
173901	2	410649	13	NULL	NULL	0	NULL	proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolation of individual proteins from whey would allow production of more consistent and reliable products by the food industry and possibly would also increase their use in the pharmaceutical industry .
	manualset3
173902	3	410649	13	NULL	NULL	0	NULL	whey 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolation of individual proteins from whey would allow production of more consistent and reliable products by the food industry and possibly would also increase their use in the pharmaceutical industry .
	manualset3
173903	4	410649	13	NULL	NULL	0	NULL	production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolation of individual proteins from whey would allow production of more consistent and reliable products by the food industry and possibly would also increase their use in the pharmaceutical industry .
	manualset3
173904	5	410649	13	NULL	NULL	0	NULL	reliable products	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolation of individual proteins from whey would allow production of more consistent and reliable products by the food industry and possibly would also increase their use in the pharmaceutical industry .
	manualset3
173905	6	410649	13	NULL	NULL	NULL	NULL	food industry	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The isolation of individual proteins from whey would allow production of more consistent and reliable products by the food industry and possibly would also increase their use in the pharmaceutical industry .
	manualset3
173906	7	410649	13	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolation of individual proteins from whey would allow production of more consistent and reliable products by the food industry and possibly would also increase their use in the pharmaceutical industry .
	manualset3
173907	8	410649	13	NULL	NULL	NULL	NULL	pharmaceutical industry	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The isolation of individual proteins from whey would allow production of more consistent and reliable products by the food industry and possibly would also increase their use in the pharmaceutical industry .
	manualset3
173908	1	410650	13	NULL	NULL	0	NULL	isolation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolation of two peptides similar in amino acid composition to that of human beta-lipotropin is presented .
	manualset3
173909	2	410650	13	NULL	NULL	0	NULL	two peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolation of two peptides similar in amino acid composition to that of human beta-lipotropin is presented .
	manualset3
173910	3	410650	13	NULL	NULL	0	NULL	amino acid	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolation of two peptides similar in amino acid composition to that of human beta-lipotropin is presented .
	manualset3
173911	4	410650	13	NULL	NULL	0	NULL	composition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolation of two peptides similar in amino acid composition to that of human beta-lipotropin is presented .
	manualset3
173912	5	410650	13	NULL	NULL	0	NULL	human beta-lipotropin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolation of two peptides similar in amino acid composition to that of human beta-lipotropin is presented .
	manualset3
173913	1	410651	13	NULL	NULL	0	NULL	jejunal motor response 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The jejunal motor response to gastric distension has been quantified in the conscious dog and compared with that of feeding in order to determine the role of the physical bulk of a meal in the conversion from fasted to fed motor activity .
	manualset3
173914	2	410651	13	NULL	NULL	0	NULL	gastric distension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The jejunal motor response to gastric distension has been quantified in the conscious dog and compared with that of feeding in order to determine the role of the physical bulk of a meal in the conversion from fasted to fed motor activity .
	manualset3
173915	3	410651	13	NULL	NULL	0	NULL	dog	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The jejunal motor response to gastric distension has been quantified in the conscious dog and compared with that of feeding in order to determine the role of the physical bulk of a meal in the conversion from fasted to fed motor activity .
	manualset3
173916	4	410651	13	NULL	NULL	0	NULL	feeding 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The jejunal motor response to gastric distension has been quantified in the conscious dog and compared with that of feeding in order to determine the role of the physical bulk of a meal in the conversion from fasted to fed motor activity .
	manualset3
173917	5	410651	13	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The jejunal motor response to gastric distension has been quantified in the conscious dog and compared with that of feeding in order to determine the role of the physical bulk of a meal in the conversion from fasted to fed motor activity .
	manualset3
173918	6	410651	13	NULL	NULL	0	NULL	physical bulk	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The jejunal motor response to gastric distension has been quantified in the conscious dog and compared with that of feeding in order to determine the role of the physical bulk of a meal in the conversion from fasted to fed motor activity .
	manualset3
173919	7	410651	13	NULL	NULL	0	NULL	meal	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The jejunal motor response to gastric distension has been quantified in the conscious dog and compared with that of feeding in order to determine the role of the physical bulk of a meal in the conversion from fasted to fed motor activity .
	manualset3
173920	8	410651	13	NULL	NULL	0	NULL	conversion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The jejunal motor response to gastric distension has been quantified in the conscious dog and compared with that of feeding in order to determine the role of the physical bulk of a meal in the conversion from fasted to fed motor activity .
	manualset3
173921	9	410651	13	NULL	NULL	0	NULL	fasted motor activity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The jejunal motor response to gastric distension has been quantified in the conscious dog and compared with that of feeding in order to determine the role of the physical bulk of a meal in the conversion from fasted to fed motor activity .
	manualset3
173922	10	410651	13	NULL	NULL	0	NULL	fed motor activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The jejunal motor response to gastric distension has been quantified in the conscious dog and compared with that of feeding in order to determine the role of the physical bulk of a meal in the conversion from fasted to fed motor activity .
	manualset3
173923	1	410652	13	NULL	NULL	0	NULL	k2 Mdh1-n y20 chromosomal region	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The k2 Mdh1-n y20 chromosomal region was very close to Satt314 , Satt253 , and Satt279 .
	manualset3
173924	2	410652	13	NULL	NULL	0	NULL	Satt314	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The k2 Mdh1-n y20 chromosomal region was very close to Satt314 , Satt253 , and Satt279 .
	manualset3
173925	3	410652	13	NULL	NULL	0	NULL	Satt253	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The k2 Mdh1-n y20 chromosomal region was very close to Satt314 , Satt253 , and Satt279 .
	manualset3
173926	4	410652	13	NULL	NULL	0	NULL	Satt279	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The k2 Mdh1-n y20 chromosomal region was very close to Satt314 , Satt253 , and Satt279 .
	manualset3
173927	1	410653	13	NULL	NULL	0	NULL	katG UAR	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The katG UAR was also able to increase expression from the Mycobacterium paratuberculosis P ( AN ) promoter 15-fold in E. coli and 12-fold in M. smegmatis .
	manualset3
173928	2	410653	13	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The katG UAR was also able to increase expression from the Mycobacterium paratuberculosis P ( AN ) promoter 15-fold in E. coli and 12-fold in M. smegmatis .
	manualset3
173929	3	410653	13	NULL	NULL	0	NULL	 Mycobacterium paratuberculosis P ( AN ) promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The katG UAR was also able to increase expression from the Mycobacterium paratuberculosis P ( AN ) promoter 15-fold in E. coli and 12-fold in M. smegmatis .
	manualset3
173930	4	410653	13	NULL	NULL	0	NULL	15-fold	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The katG UAR was also able to increase expression from the Mycobacterium paratuberculosis P ( AN ) promoter 15-fold in E. coli and 12-fold in M. smegmatis .
	manualset3
173931	5	410653	13	NULL	NULL	0	NULL	E. coli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The katG UAR was also able to increase expression from the Mycobacterium paratuberculosis P ( AN ) promoter 15-fold in E. coli and 12-fold in M. smegmatis .
	manualset3
173932	6	410653	13	NULL	NULL	0	NULL	12-fold	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The katG UAR was also able to increase expression from the Mycobacterium paratuberculosis P ( AN ) promoter 15-fold in E. coli and 12-fold in M. smegmatis .
	manualset3
173933	7	410653	13	NULL	NULL	0	NULL	M. smegmatis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The katG UAR was also able to increase expression from the Mycobacterium paratuberculosis P ( AN ) promoter 15-fold in E. coli and 12-fold in M. smegmatis .
	manualset3
173934	1	410654	13	NULL	NULL	NULL	NULL	keratin K8	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The keratin K8 and K19 reactivity was retained in those chordomas showing solid sheets of epithelioid , spindle cells , or cartilaginous metaplasia , and in one of two cases showing overtly sarcomatous transformation .
	manualset3
173935	2	410654	13	NULL	NULL	0	NULL	keratin K19	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The keratin K8 and K19 reactivity was retained in those chordomas showing solid sheets of epithelioid , spindle cells , or cartilaginous metaplasia , and in one of two cases showing overtly sarcomatous transformation .
	manualset3
173936	3	410654	13	NULL	NULL	0	NULL	reactivity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The keratin K8 and K19 reactivity was retained in those chordomas showing solid sheets of epithelioid , spindle cells , or cartilaginous metaplasia , and in one of two cases showing overtly sarcomatous transformation .
	manualset3
173937	4	410654	13	NULL	NULL	0	NULL	chordomas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The keratin K8 and K19 reactivity was retained in those chordomas showing solid sheets of epithelioid , spindle cells , or cartilaginous metaplasia , and in one of two cases showing overtly sarcomatous transformation .
	manualset3
173938	5	410654	13	NULL	NULL	0	NULL	solid sheets 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The keratin K8 and K19 reactivity was retained in those chordomas showing solid sheets of epithelioid , spindle cells , or cartilaginous metaplasia , and in one of two cases showing overtly sarcomatous transformation .
	manualset3
173939	6	410654	13	NULL	NULL	0	NULL	epithelioid cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The keratin K8 and K19 reactivity was retained in those chordomas showing solid sheets of epithelioid , spindle cells , or cartilaginous metaplasia , and in one of two cases showing overtly sarcomatous transformation .
	manualset3
173940	7	410654	13	NULL	NULL	0	NULL	spindle cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The keratin K8 and K19 reactivity was retained in those chordomas showing solid sheets of epithelioid , spindle cells , or cartilaginous metaplasia , and in one of two cases showing overtly sarcomatous transformation .
	manualset3
173941	8	410654	13	NULL	NULL	0	NULL	cartilaginous metaplasia	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The keratin K8 and K19 reactivity was retained in those chordomas showing solid sheets of epithelioid , spindle cells , or cartilaginous metaplasia , and in one of two cases showing overtly sarcomatous transformation .
	manualset3
173942	9	410654	13	NULL	NULL	0	NULL	one 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The keratin K8 and K19 reactivity was retained in those chordomas showing solid sheets of epithelioid , spindle cells , or cartilaginous metaplasia , and in one of two cases showing overtly sarcomatous transformation .
	manualset3
173944	10	410654	13	NULL	NULL	0	NULL	two cases	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The keratin K8 and K19 reactivity was retained in those chordomas showing solid sheets of epithelioid , spindle cells , or cartilaginous metaplasia , and in one of two cases showing overtly sarcomatous transformation .
	manualset3
173945	11	410654	13	NULL	NULL	0	NULL	sarcomatous transformation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The keratin K8 and K19 reactivity was retained in those chordomas showing solid sheets of epithelioid , spindle cells , or cartilaginous metaplasia , and in one of two cases showing overtly sarcomatous transformation .
	manualset3
173946	1	410655	13	NULL	NULL	NULL	NULL	key	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The key collective structural variable that plays the role of the dynamic order parameter for aging is the experimentally measurable nanometer and longer wavelength amplitude of density fluctuations , S0 .
	manualset3
173951	2	410655	13	NULL	NULL	0	NULL	variable	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The key collective structural variable that plays the role of the dynamic order parameter for aging is the experimentally measurable nanometer and longer wavelength amplitude of density fluctuations , S0 .
	manualset3
173952	3	410655	13	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The key collective structural variable that plays the role of the dynamic order parameter for aging is the experimentally measurable nanometer and longer wavelength amplitude of density fluctuations , S0 .
	manualset3
173953	4	410655	13	NULL	NULL	0	NULL	dynamic order parameter 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The key collective structural variable that plays the role of the dynamic order parameter for aging is the experimentally measurable nanometer and longer wavelength amplitude of density fluctuations , S0 .
	manualset3
173954	5	410655	13	NULL	NULL	0	NULL	nanometer	Unit												NULL		0	NULL	NULL	NULL	NULL	NULL	The key collective structural variable that plays the role of the dynamic order parameter for aging is the experimentally measurable nanometer and longer wavelength amplitude of density fluctuations , S0 .
	manualset3
173955	6	410655	13	NULL	NULL	0	NULL	wavelength amplitude 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The key collective structural variable that plays the role of the dynamic order parameter for aging is the experimentally measurable nanometer and longer wavelength amplitude of density fluctuations , S0 .
	manualset3
173956	7	410655	13	NULL	NULL	0	NULL	density fluctuations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The key collective structural variable that plays the role of the dynamic order parameter for aging is the experimentally measurable nanometer and longer wavelength amplitude of density fluctuations , S0 .
	manualset3
173957	8	410655	13	NULL	NULL	0	NULL	S0 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The key collective structural variable that plays the role of the dynamic order parameter for aging is the experimentally measurable nanometer and longer wavelength amplitude of density fluctuations , S0 .
	manualset3
173958	1	410656	13	NULL	NULL	0	NULL	key intermediate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The key intermediate , 15-oxandrost-5-en-3 beta , 17 beta-diyl 3-acetate 17-benzoate ( 10 ) , was prepared by a five-step procedure based on the addition of 4-methoxybenzyl alcohol to 3 beta-hydroxyandrosta-5 , 15-dien-17-one ( 1 ) .
	manualset3
173959	2	410656	13	NULL	NULL	0	NULL	15-oxandrost-5-en-3 beta , 17 beta-diyl 3-acetate 17-benzoate ( 10 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The key intermediate , 15-oxandrost-5-en-3 beta , 17 beta-diyl 3-acetate 17-benzoate ( 10 ) , was prepared by a five-step procedure based on the addition of 4-methoxybenzyl alcohol to 3 beta-hydroxyandrosta-5 , 15-dien-17-one ( 1 ) .
	manualset3
173960	3	410656	13	NULL	NULL	0	NULL	five-step procedure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The key intermediate , 15-oxandrost-5-en-3 beta , 17 beta-diyl 3-acetate 17-benzoate ( 10 ) , was prepared by a five-step procedure based on the addition of 4-methoxybenzyl alcohol to 3 beta-hydroxyandrosta-5 , 15-dien-17-one ( 1 ) .
	manualset3
173961	4	410656	13	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The key intermediate , 15-oxandrost-5-en-3 beta , 17 beta-diyl 3-acetate 17-benzoate ( 10 ) , was prepared by a five-step procedure based on the addition of 4-methoxybenzyl alcohol to 3 beta-hydroxyandrosta-5 , 15-dien-17-one ( 1 ) .
	manualset3
173962	5	410656	13	NULL	NULL	0	NULL	4-methoxybenzyl alcohol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The key intermediate , 15-oxandrost-5-en-3 beta , 17 beta-diyl 3-acetate 17-benzoate ( 10 ) , was prepared by a five-step procedure based on the addition of 4-methoxybenzyl alcohol to 3 beta-hydroxyandrosta-5 , 15-dien-17-one ( 1 ) .
	manualset3
173963	6	410656	13	NULL	NULL	0	NULL	3 beta-hydroxyandrosta-5 , 15-dien-17-one ( 1 ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The key intermediate , 15-oxandrost-5-en-3 beta , 17 beta-diyl 3-acetate 17-benzoate ( 10 ) , was prepared by a five-step procedure based on the addition of 4-methoxybenzyl alcohol to 3 beta-hydroxyandrosta-5 , 15-dien-17-one ( 1 ) .
	manualset3
173964	1	410657	13	NULL	NULL	0	NULL	killer molecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The killer molecule of complement .
	manualset3
173965	2	410657	13	NULL	NULL	0	NULL	complement	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The killer molecule of complement .
	manualset3
173990	1	410658	13	NULL	NULL	0	NULL	killing-effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The killing-effect was not revealed when the lymphoid cells were obtained from the donors on the 30th day after irradiation .
	manualset3
173993	2	410658	13	NULL	NULL	0	NULL	lymphoid cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The killing-effect was not revealed when the lymphoid cells were obtained from the donors on the 30th day after irradiation .
	manualset3
173994	3	410658	13	NULL	NULL	0	NULL	donors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The killing-effect was not revealed when the lymphoid cells were obtained from the donors on the 30th day after irradiation .
	manualset3
173995	4	410658	13	NULL	NULL	0	NULL	30th day	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The killing-effect was not revealed when the lymphoid cells were obtained from the donors on the 30th day after irradiation .
	manualset3
173996	5	410658	13	NULL	NULL	0	NULL	irradiation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The killing-effect was not revealed when the lymphoid cells were obtained from the donors on the 30th day after irradiation .
	manualset3
173997	1	410659	13	NULL	NULL	0	NULL	kinetic data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetic data of the compounds were compared to those of the metoprolol and ASA control periods .
	manualset3
173998	2	410659	13	NULL	NULL	0	NULL	compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetic data of the compounds were compared to those of the metoprolol and ASA control periods .
	manualset3
173999	3	410659	13	NULL	NULL	0	NULL	metoprolol 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetic data of the compounds were compared to those of the metoprolol and ASA control periods .
	manualset3
174000	4	410659	13	NULL	NULL	0	NULL	ASA	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetic data of the compounds were compared to those of the metoprolol and ASA control periods .
	manualset3
174001	5	410659	13	NULL	NULL	0	NULL	control periods	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetic data of the compounds were compared to those of the metoprolol and ASA control periods .
	manualset3
174002	1	410660	13	NULL	NULL	0	NULL	kinetics	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of cytolysis was NK-like , with maximal 51Cr-release within 4-8 hours of co-culture , and with a high degree of methyl-3H-thymidine release during the first 24 hour of co-culture , and with a high degree of methyl-3H-thymidine release during the first 24 hours of co-culture .
	manualset3
174003	2	410660	13	NULL	NULL	0	NULL	cytolysis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of cytolysis was NK-like , with maximal 51Cr-release within 4-8 hours of co-culture , and with a high degree of methyl-3H-thymidine release during the first 24 hour of co-culture , and with a high degree of methyl-3H-thymidine release during the first 24 hours of co-culture .
	manualset3
174004	3	410660	13	NULL	NULL	0	NULL	51Cr-release 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of cytolysis was NK-like , with maximal 51Cr-release within 4-8 hours of co-culture , and with a high degree of methyl-3H-thymidine release during the first 24 hour of co-culture , and with a high degree of methyl-3H-thymidine release during the first 24 hours of co-culture .
	manualset3
174005	4	410660	13	NULL	NULL	0	NULL	4-8 hours 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of cytolysis was NK-like , with maximal 51Cr-release within 4-8 hours of co-culture , and with a high degree of methyl-3H-thymidine release during the first 24 hour of co-culture , and with a high degree of methyl-3H-thymidine release during the first 24 hours of co-culture .
	manualset3
174006	5	410660	13	NULL	NULL	0	NULL	co-culture	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of cytolysis was NK-like , with maximal 51Cr-release within 4-8 hours of co-culture , and with a high degree of methyl-3H-thymidine release during the first 24 hour of co-culture , and with a high degree of methyl-3H-thymidine release during the first 24 hours of co-culture .
	manualset3
174007	6	410660	13	NULL	NULL	0	NULL	high degree 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of cytolysis was NK-like , with maximal 51Cr-release within 4-8 hours of co-culture , and with a high degree of methyl-3H-thymidine release during the first 24 hour of co-culture , and with a high degree of methyl-3H-thymidine release during the first 24 hours of co-culture .
	manualset3
174008	7	410660	13	NULL	NULL	0	NULL	methyl-3H-thymidine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of cytolysis was NK-like , with maximal 51Cr-release within 4-8 hours of co-culture , and with a high degree of methyl-3H-thymidine release during the first 24 hour of co-culture , and with a high degree of methyl-3H-thymidine release during the first 24 hours of co-culture .
	manualset3
174009	8	410660	13	NULL	NULL	0	NULL	release 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of cytolysis was NK-like , with maximal 51Cr-release within 4-8 hours of co-culture , and with a high degree of methyl-3H-thymidine release during the first 24 hour of co-culture , and with a high degree of methyl-3H-thymidine release during the first 24 hours of co-culture .
	manualset3
174010	9	410660	13	NULL	NULL	0	NULL	first 24 hour	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of cytolysis was NK-like , with maximal 51Cr-release within 4-8 hours of co-culture , and with a high degree of methyl-3H-thymidine release during the first 24 hour of co-culture , and with a high degree of methyl-3H-thymidine release during the first 24 hours of co-culture .
	manualset3
174011	10	410660	13	NULL	NULL	0	NULL	co-culture 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of cytolysis was NK-like , with maximal 51Cr-release within 4-8 hours of co-culture , and with a high degree of methyl-3H-thymidine release during the first 24 hour of co-culture , and with a high degree of methyl-3H-thymidine release during the first 24 hours of co-culture .
	manualset3
174012	11	410660	13	NULL	NULL	0	NULL	high degree	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of cytolysis was NK-like , with maximal 51Cr-release within 4-8 hours of co-culture , and with a high degree of methyl-3H-thymidine release during the first 24 hour of co-culture , and with a high degree of methyl-3H-thymidine release during the first 24 hours of co-culture .
	manualset3
174013	12	410660	13	NULL	NULL	0	NULL	methyl-3H-thymidine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of cytolysis was NK-like , with maximal 51Cr-release within 4-8 hours of co-culture , and with a high degree of methyl-3H-thymidine release during the first 24 hour of co-culture , and with a high degree of methyl-3H-thymidine release during the first 24 hours of co-culture .
	manualset3
174014	13	410660	13	NULL	NULL	0	NULL	release	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of cytolysis was NK-like , with maximal 51Cr-release within 4-8 hours of co-culture , and with a high degree of methyl-3H-thymidine release during the first 24 hour of co-culture , and with a high degree of methyl-3H-thymidine release during the first 24 hours of co-culture .
	manualset3
174015	14	410660	13	NULL	NULL	0	NULL	first 24 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of cytolysis was NK-like , with maximal 51Cr-release within 4-8 hours of co-culture , and with a high degree of methyl-3H-thymidine release during the first 24 hour of co-culture , and with a high degree of methyl-3H-thymidine release during the first 24 hours of co-culture .
	manualset3
174016	15	410660	13	NULL	NULL	0	NULL	co-culture	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of cytolysis was NK-like , with maximal 51Cr-release within 4-8 hours of co-culture , and with a high degree of methyl-3H-thymidine release during the first 24 hour of co-culture , and with a high degree of methyl-3H-thymidine release during the first 24 hours of co-culture .
	manualset3
174017	1	410661	13	NULL	NULL	0	NULL	kinetics 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of enzyme carbamylation with N-methyl ( 7-dimethylcarbamoxy ) quinolinium iodide was studied in single-turnover conditions up to 1.2 kbar using a high-pressure stopped-flow fluorimeter .
	manualset3
174018	2	410661	13	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of enzyme carbamylation with N-methyl ( 7-dimethylcarbamoxy ) quinolinium iodide was studied in single-turnover conditions up to 1.2 kbar using a high-pressure stopped-flow fluorimeter .
	manualset3
174019	3	410661	13	NULL	NULL	0	NULL	carbamylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of enzyme carbamylation with N-methyl ( 7-dimethylcarbamoxy ) quinolinium iodide was studied in single-turnover conditions up to 1.2 kbar using a high-pressure stopped-flow fluorimeter .
	manualset3
174020	4	410661	13	NULL	NULL	0	NULL	N-methyl ( 7-dimethylcarbamoxy ) quinolinium iodide 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of enzyme carbamylation with N-methyl ( 7-dimethylcarbamoxy ) quinolinium iodide was studied in single-turnover conditions up to 1.2 kbar using a high-pressure stopped-flow fluorimeter .
	manualset3
174021	5	410661	13	NULL	NULL	0	NULL	single-turnover conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of enzyme carbamylation with N-methyl ( 7-dimethylcarbamoxy ) quinolinium iodide was studied in single-turnover conditions up to 1.2 kbar using a high-pressure stopped-flow fluorimeter .
	manualset3
174022	6	410661	13	NULL	NULL	0	NULL	1.2 kbar	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of enzyme carbamylation with N-methyl ( 7-dimethylcarbamoxy ) quinolinium iodide was studied in single-turnover conditions up to 1.2 kbar using a high-pressure stopped-flow fluorimeter .
	manualset3
174023	7	410661	13	NULL	NULL	0	NULL	high-pressure stopped-flow fluorimeter	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of enzyme carbamylation with N-methyl ( 7-dimethylcarbamoxy ) quinolinium iodide was studied in single-turnover conditions up to 1.2 kbar using a high-pressure stopped-flow fluorimeter .
	manualset3
174044	1	410662	13	NULL	NULL	0	NULL	kinetics 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of the formation of the metaII ( MII ) state of bovine rhodopsin was investigated by time-resolved electrical and absorption measurements with rod outer segment ( ROS ) fragments .
	manualset3
174045	2	410662	13	NULL	NULL	0	NULL	formation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of the formation of the metaII ( MII ) state of bovine rhodopsin was investigated by time-resolved electrical and absorption measurements with rod outer segment ( ROS ) fragments .
	manualset3
174046	3	410662	13	NULL	NULL	0	NULL	metaII ( MII ) state	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of the formation of the metaII ( MII ) state of bovine rhodopsin was investigated by time-resolved electrical and absorption measurements with rod outer segment ( ROS ) fragments .
	manualset3
174047	4	410662	13	NULL	NULL	0	NULL	bovine rhodopsin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of the formation of the metaII ( MII ) state of bovine rhodopsin was investigated by time-resolved electrical and absorption measurements with rod outer segment ( ROS ) fragments .
	manualset3
174048	5	410662	13	NULL	NULL	NULL	NULL	electrical measurements	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The kinetics of the formation of the metaII ( MII ) state of bovine rhodopsin was investigated by time-resolved electrical and absorption measurements with rod outer segment ( ROS ) fragments .
	manualset3
174049	6	410662	13	NULL	NULL	0	NULL	absorption measurements	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of the formation of the metaII ( MII ) state of bovine rhodopsin was investigated by time-resolved electrical and absorption measurements with rod outer segment ( ROS ) fragments .
	manualset3
174050	7	410662	13	NULL	NULL	0	NULL	rod outer segment ( ROS ) fragments	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of the formation of the metaII ( MII ) state of bovine rhodopsin was investigated by time-resolved electrical and absorption measurements with rod outer segment ( ROS ) fragments .
	manualset3
174051	1	410663	13	NULL	NULL	0	NULL	knowledge	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The knowledge that gastrointestinal cancers can calcify and ossify has a definite diagnostic relevance for the radiologist and gastroenterologist .
	manualset3
174052	2	410663	13	NULL	NULL	0	NULL	gastrointestinal cancers 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The knowledge that gastrointestinal cancers can calcify and ossify has a definite diagnostic relevance for the radiologist and gastroenterologist .
	manualset3
174053	3	410663	13	NULL	NULL	0	NULL	diagnostic relevance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The knowledge that gastrointestinal cancers can calcify and ossify has a definite diagnostic relevance for the radiologist and gastroenterologist .
	manualset3
174054	4	410663	13	NULL	NULL	0	NULL	radiologist	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The knowledge that gastrointestinal cancers can calcify and ossify has a definite diagnostic relevance for the radiologist and gastroenterologist .
	manualset3
174055	5	410663	13	NULL	NULL	0	NULL	gastroenterologist	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The knowledge that gastrointestinal cancers can calcify and ossify has a definite diagnostic relevance for the radiologist and gastroenterologist .
	manualset3
174056	1	410664	13	NULL	NULL	0	NULL	label 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The label penetrates into the interstitium and is accumulated in the activated macrophages .
	manualset3
174057	2	410664	13	NULL	NULL	0	NULL	interstitium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The label penetrates into the interstitium and is accumulated in the activated macrophages .
	manualset3
174058	3	410664	13	NULL	NULL	0	NULL	macrophages 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The label penetrates into the interstitium and is accumulated in the activated macrophages .
	manualset3
174059	1	410665	13	NULL	NULL	0	NULL	ligand	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The labeled ligand is prepared by a stoichiometric iodination procedure in which one atom of iodine-125 is incorporated into one molecule of the hormone , resulting in an intact labeled prolactin with a high specific activity of 170-186 muCi/micrograms ( 1 Ci = 37 GBq ) .
	manualset3
174060	2	410665	13	NULL	NULL	NULL	NULL	 stoichiometric iodination procedure	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The labeled ligand is prepared by a stoichiometric iodination procedure in which one atom of iodine-125 is incorporated into one molecule of the hormone , resulting in an intact labeled prolactin with a high specific activity of 170-186 muCi/micrograms ( 1 Ci = 37 GBq ) .
	manualset3
174061	3	410665	13	NULL	NULL	0	NULL	one atom	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The labeled ligand is prepared by a stoichiometric iodination procedure in which one atom of iodine-125 is incorporated into one molecule of the hormone , resulting in an intact labeled prolactin with a high specific activity of 170-186 muCi/micrograms ( 1 Ci = 37 GBq ) .
	manualset3
174062	4	410665	13	NULL	NULL	0	NULL	iodine-125	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The labeled ligand is prepared by a stoichiometric iodination procedure in which one atom of iodine-125 is incorporated into one molecule of the hormone , resulting in an intact labeled prolactin with a high specific activity of 170-186 muCi/micrograms ( 1 Ci = 37 GBq ) .
	manualset3
174063	5	410665	13	NULL	NULL	0	NULL	one molecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The labeled ligand is prepared by a stoichiometric iodination procedure in which one atom of iodine-125 is incorporated into one molecule of the hormone , resulting in an intact labeled prolactin with a high specific activity of 170-186 muCi/micrograms ( 1 Ci = 37 GBq ) .
	manualset3
174064	6	410665	13	NULL	NULL	0	NULL	hormone	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The labeled ligand is prepared by a stoichiometric iodination procedure in which one atom of iodine-125 is incorporated into one molecule of the hormone , resulting in an intact labeled prolactin with a high specific activity of 170-186 muCi/micrograms ( 1 Ci = 37 GBq ) .
	manualset3
174065	7	410665	13	NULL	NULL	0	NULL	prolactin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The labeled ligand is prepared by a stoichiometric iodination procedure in which one atom of iodine-125 is incorporated into one molecule of the hormone , resulting in an intact labeled prolactin with a high specific activity of 170-186 muCi/micrograms ( 1 Ci = 37 GBq ) .
	manualset3
174066	8	410665	13	NULL	NULL	0	NULL	high specific activity 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The labeled ligand is prepared by a stoichiometric iodination procedure in which one atom of iodine-125 is incorporated into one molecule of the hormone , resulting in an intact labeled prolactin with a high specific activity of 170-186 muCi/micrograms ( 1 Ci = 37 GBq ) .
	manualset3
174067	9	410665	13	NULL	NULL	NULL	NULL	 170-186 muCi/micrograms 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The labeled ligand is prepared by a stoichiometric iodination procedure in which one atom of iodine-125 is incorporated into one molecule of the hormone , resulting in an intact labeled prolactin with a high specific activity of 170-186 muCi/micrograms ( 1 Ci = 37 GBq ) .
	manualset3
174068	10	410665	13	NULL	NULL	0	NULL	1 Ci = 37 GBq	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The labeled ligand is prepared by a stoichiometric iodination procedure in which one atom of iodine-125 is incorporated into one molecule of the hormone , resulting in an intact labeled prolactin with a high specific activity of 170-186 muCi/micrograms ( 1 Ci = 37 GBq ) .
	manualset3
174069	1	410666	13	NULL	NULL	0	NULL	total	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 3 , 653 residents randomly selected from among the citizens of Suita City , Osaka , Japan were enlisted as subjects , in whom we investigated sweet preference , clinical characteristics , including obesity and serum leptin level , and the polymorphisms of LEP and LEPR ( G-2548A and A19G for LEP ; R109K , R223Q , and rs3790439 for LEPR ) .
	manualset3
174070	2	410666	13	NULL	NULL	0	NULL	3 , 653 residents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 3 , 653 residents randomly selected from among the citizens of Suita City , Osaka , Japan were enlisted as subjects , in whom we investigated sweet preference , clinical characteristics , including obesity and serum leptin level , and the polymorphisms of LEP and LEPR ( G-2548A and A19G for LEP ; R109K , R223Q , and rs3790439 for LEPR ) .
	manualset3
174071	3	410666	13	NULL	NULL	0	NULL	citizens	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 3 , 653 residents randomly selected from among the citizens of Suita City , Osaka , Japan were enlisted as subjects , in whom we investigated sweet preference , clinical characteristics , including obesity and serum leptin level , and the polymorphisms of LEP and LEPR ( G-2548A and A19G for LEP ; R109K , R223Q , and rs3790439 for LEPR ) .
	manualset3
174072	4	410666	13	NULL	NULL	0	NULL	Suita City	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 3 , 653 residents randomly selected from among the citizens of Suita City , Osaka , Japan were enlisted as subjects , in whom we investigated sweet preference , clinical characteristics , including obesity and serum leptin level , and the polymorphisms of LEP and LEPR ( G-2548A and A19G for LEP ; R109K , R223Q , and rs3790439 for LEPR ) .
	manualset3
174073	5	410666	13	NULL	NULL	0	NULL	Osaka	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 3 , 653 residents randomly selected from among the citizens of Suita City , Osaka , Japan were enlisted as subjects , in whom we investigated sweet preference , clinical characteristics , including obesity and serum leptin level , and the polymorphisms of LEP and LEPR ( G-2548A and A19G for LEP ; R109K , R223Q , and rs3790439 for LEPR ) .
	manualset3
174074	6	410666	13	NULL	NULL	0	NULL	Japan	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 3 , 653 residents randomly selected from among the citizens of Suita City , Osaka , Japan were enlisted as subjects , in whom we investigated sweet preference , clinical characteristics , including obesity and serum leptin level , and the polymorphisms of LEP and LEPR ( G-2548A and A19G for LEP ; R109K , R223Q , and rs3790439 for LEPR ) .
	manualset3
174075	7	410666	13	NULL	NULL	0	NULL	subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 3 , 653 residents randomly selected from among the citizens of Suita City , Osaka , Japan were enlisted as subjects , in whom we investigated sweet preference , clinical characteristics , including obesity and serum leptin level , and the polymorphisms of LEP and LEPR ( G-2548A and A19G for LEP ; R109K , R223Q , and rs3790439 for LEPR ) .
	manualset3
174076	8	410666	13	NULL	NULL	NULL	NULL	sweet preference	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A total of 3 , 653 residents randomly selected from among the citizens of Suita City , Osaka , Japan were enlisted as subjects , in whom we investigated sweet preference , clinical characteristics , including obesity and serum leptin level , and the polymorphisms of LEP and LEPR ( G-2548A and A19G for LEP ; R109K , R223Q , and rs3790439 for LEPR ) .
	manualset3
174077	9	410666	13	NULL	NULL	0	NULL	clinical characteristics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 3 , 653 residents randomly selected from among the citizens of Suita City , Osaka , Japan were enlisted as subjects , in whom we investigated sweet preference , clinical characteristics , including obesity and serum leptin level , and the polymorphisms of LEP and LEPR ( G-2548A and A19G for LEP ; R109K , R223Q , and rs3790439 for LEPR ) .
	manualset3
174078	10	410666	13	NULL	NULL	0	NULL	obesity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 3 , 653 residents randomly selected from among the citizens of Suita City , Osaka , Japan were enlisted as subjects , in whom we investigated sweet preference , clinical characteristics , including obesity and serum leptin level , and the polymorphisms of LEP and LEPR ( G-2548A and A19G for LEP ; R109K , R223Q , and rs3790439 for LEPR ) .
	manualset3
174079	11	410666	13	NULL	NULL	0	NULL	serum leptin level 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 3 , 653 residents randomly selected from among the citizens of Suita City , Osaka , Japan were enlisted as subjects , in whom we investigated sweet preference , clinical characteristics , including obesity and serum leptin level , and the polymorphisms of LEP and LEPR ( G-2548A and A19G for LEP ; R109K , R223Q , and rs3790439 for LEPR ) .
	manualset3
174080	12	410666	13	NULL	NULL	0	NULL	polymorphisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 3 , 653 residents randomly selected from among the citizens of Suita City , Osaka , Japan were enlisted as subjects , in whom we investigated sweet preference , clinical characteristics , including obesity and serum leptin level , and the polymorphisms of LEP and LEPR ( G-2548A and A19G for LEP ; R109K , R223Q , and rs3790439 for LEPR ) .
	manualset3
174081	13	410666	13	NULL	NULL	0	NULL	 LEP 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 3 , 653 residents randomly selected from among the citizens of Suita City , Osaka , Japan were enlisted as subjects , in whom we investigated sweet preference , clinical characteristics , including obesity and serum leptin level , and the polymorphisms of LEP and LEPR ( G-2548A and A19G for LEP ; R109K , R223Q , and rs3790439 for LEPR ) .
	manualset3
174082	14	410666	13	NULL	NULL	0	NULL	LEPR	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 3 , 653 residents randomly selected from among the citizens of Suita City , Osaka , Japan were enlisted as subjects , in whom we investigated sweet preference , clinical characteristics , including obesity and serum leptin level , and the polymorphisms of LEP and LEPR ( G-2548A and A19G for LEP ; R109K , R223Q , and rs3790439 for LEPR ) .
	manualset3
174083	15	410666	13	NULL	NULL	NULL	NULL	G-2548A	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A total of 3 , 653 residents randomly selected from among the citizens of Suita City , Osaka , Japan were enlisted as subjects , in whom we investigated sweet preference , clinical characteristics , including obesity and serum leptin level , and the polymorphisms of LEP and LEPR ( G-2548A and A19G for LEP ; R109K , R223Q , and rs3790439 for LEPR ) .
	manualset3
174084	16	410666	13	NULL	NULL	0	NULL	A19G	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 3 , 653 residents randomly selected from among the citizens of Suita City , Osaka , Japan were enlisted as subjects , in whom we investigated sweet preference , clinical characteristics , including obesity and serum leptin level , and the polymorphisms of LEP and LEPR ( G-2548A and A19G for LEP ; R109K , R223Q , and rs3790439 for LEPR ) .
	manualset3
174085	17	410666	13	NULL	NULL	0	NULL	LEP	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 3 , 653 residents randomly selected from among the citizens of Suita City , Osaka , Japan were enlisted as subjects , in whom we investigated sweet preference , clinical characteristics , including obesity and serum leptin level , and the polymorphisms of LEP and LEPR ( G-2548A and A19G for LEP ; R109K , R223Q , and rs3790439 for LEPR ) .
	manualset3
174086	18	410666	13	NULL	NULL	0	NULL	R109K	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 3 , 653 residents randomly selected from among the citizens of Suita City , Osaka , Japan were enlisted as subjects , in whom we investigated sweet preference , clinical characteristics , including obesity and serum leptin level , and the polymorphisms of LEP and LEPR ( G-2548A and A19G for LEP ; R109K , R223Q , and rs3790439 for LEPR ) .
	manualset3
174087	19	410666	13	NULL	NULL	0	NULL	R223Q	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 3 , 653 residents randomly selected from among the citizens of Suita City , Osaka , Japan were enlisted as subjects , in whom we investigated sweet preference , clinical characteristics , including obesity and serum leptin level , and the polymorphisms of LEP and LEPR ( G-2548A and A19G for LEP ; R109K , R223Q , and rs3790439 for LEPR ) .
	manualset3
174088	20	410666	13	NULL	NULL	0	NULL	rs3790439	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 3 , 653 residents randomly selected from among the citizens of Suita City , Osaka , Japan were enlisted as subjects , in whom we investigated sweet preference , clinical characteristics , including obesity and serum leptin level , and the polymorphisms of LEP and LEPR ( G-2548A and A19G for LEP ; R109K , R223Q , and rs3790439 for LEPR ) .
	manualset3
174089	21	410666	13	NULL	NULL	0	NULL	LEPR	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 3 , 653 residents randomly selected from among the citizens of Suita City , Osaka , Japan were enlisted as subjects , in whom we investigated sweet preference , clinical characteristics , including obesity and serum leptin level , and the polymorphisms of LEP and LEPR ( G-2548A and A19G for LEP ; R109K , R223Q , and rs3790439 for LEPR ) .
	manualset3
174090	1	410667	13	NULL	NULL	0	NULL	N-glycans	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The labeled N-glycans were separated into neutral and charged fractions by anion exchange chromatography and the charged N-glycans were found to be mostly alpha2 , 6-monosialylated with Neu5Ac or Neu5Gc in a ratio of 1 : 1 .
	manualset3
174091	2	410667	13	NULL	NULL	0	NULL	neutral fractions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The labeled N-glycans were separated into neutral and charged fractions by anion exchange chromatography and the charged N-glycans were found to be mostly alpha2 , 6-monosialylated with Neu5Ac or Neu5Gc in a ratio of 1 : 1 .
	manualset3
174092	3	410667	13	NULL	NULL	0	NULL	charged fractions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The labeled N-glycans were separated into neutral and charged fractions by anion exchange chromatography and the charged N-glycans were found to be mostly alpha2 , 6-monosialylated with Neu5Ac or Neu5Gc in a ratio of 1 : 1 .
	manualset3
174093	4	410667	13	NULL	NULL	0	NULL	anion exchange chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The labeled N-glycans were separated into neutral and charged fractions by anion exchange chromatography and the charged N-glycans were found to be mostly alpha2 , 6-monosialylated with Neu5Ac or Neu5Gc in a ratio of 1 : 1 .
	manualset3
174094	5	410667	13	NULL	NULL	0	NULL	charged N-glycans 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The labeled N-glycans were separated into neutral and charged fractions by anion exchange chromatography and the charged N-glycans were found to be mostly alpha2 , 6-monosialylated with Neu5Ac or Neu5Gc in a ratio of 1 : 1 .
	manualset3
174095	6	410667	13	NULL	NULL	0	NULL	 alpha2 , 6-monosialylated with Neu5Ac	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The labeled N-glycans were separated into neutral and charged fractions by anion exchange chromatography and the charged N-glycans were found to be mostly alpha2 , 6-monosialylated with Neu5Ac or Neu5Gc in a ratio of 1 : 1 .
	manualset3
174096	7	410667	13	NULL	NULL	0	NULL	 alpha2 , 6-monosialylated with Neu5Gc	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The labeled N-glycans were separated into neutral and charged fractions by anion exchange chromatography and the charged N-glycans were found to be mostly alpha2 , 6-monosialylated with Neu5Ac or Neu5Gc in a ratio of 1 : 1 .
	manualset3
174097	8	410667	13	NULL	NULL	0	NULL	ratio	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The labeled N-glycans were separated into neutral and charged fractions by anion exchange chromatography and the charged N-glycans were found to be mostly alpha2 , 6-monosialylated with Neu5Ac or Neu5Gc in a ratio of 1 : 1 .
	manualset3
174098	9	410667	13	NULL	NULL	0	NULL	1 : 1 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The labeled N-glycans were separated into neutral and charged fractions by anion exchange chromatography and the charged N-glycans were found to be mostly alpha2 , 6-monosialylated with Neu5Ac or Neu5Gc in a ratio of 1 : 1 .
	manualset3
174099	1	410668	13	NULL	NULL	0	NULL	lack	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The lack of Ca ( V ) expression suppressed channel regulation by RIM1 .
	manualset3
174100	2	410668	13	NULL	NULL	0	NULL	Ca ( V ) expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The lack of Ca ( V ) expression suppressed channel regulation by RIM1 .
	manualset3
174101	3	410668	13	NULL	NULL	NULL	NULL	channel regulation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The lack of Ca ( V ) expression suppressed channel regulation by RIM1 .
	manualset3
174102	4	410668	13	NULL	NULL	0	NULL	RIM1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The lack of Ca ( V ) expression suppressed channel regulation by RIM1 .
	manualset3
174103	1	410669	13	NULL	NULL	0	NULL	lack 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The lack of convenient HDV infection models has hampered the development of effective therapeutics .
	manualset3
174104	2	410669	13	NULL	NULL	0	NULL	HDV infection models 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The lack of convenient HDV infection models has hampered the development of effective therapeutics .
	manualset3
174105	3	410669	13	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The lack of convenient HDV infection models has hampered the development of effective therapeutics .
	manualset3
174106	4	410669	13	NULL	NULL	0	NULL	effective therapeutics	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The lack of convenient HDV infection models has hampered the development of effective therapeutics .
	manualset3
174139	1	410670	13	NULL	NULL	0	NULL	lack	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The lack of reduction of the penultimate residue at the C-terminus may indicate that this step is normally at the end of the biosynthetic pathway of peptaibols and occurs with cleavage of Gly .
	manualset3
174140	2	410670	13	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The lack of reduction of the penultimate residue at the C-terminus may indicate that this step is normally at the end of the biosynthetic pathway of peptaibols and occurs with cleavage of Gly .
	manualset3
174141	3	410670	13	NULL	NULL	0	NULL	penultimate residue	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The lack of reduction of the penultimate residue at the C-terminus may indicate that this step is normally at the end of the biosynthetic pathway of peptaibols and occurs with cleavage of Gly .
	manualset3
174142	4	410670	13	NULL	NULL	0	NULL	C-terminus	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The lack of reduction of the penultimate residue at the C-terminus may indicate that this step is normally at the end of the biosynthetic pathway of peptaibols and occurs with cleavage of Gly .
	manualset3
174143	5	410670	13	NULL	NULL	0	NULL	step 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The lack of reduction of the penultimate residue at the C-terminus may indicate that this step is normally at the end of the biosynthetic pathway of peptaibols and occurs with cleavage of Gly .
	manualset3
174144	6	410670	13	NULL	NULL	0	NULL	end	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The lack of reduction of the penultimate residue at the C-terminus may indicate that this step is normally at the end of the biosynthetic pathway of peptaibols and occurs with cleavage of Gly .
	manualset3
174145	7	410670	13	NULL	NULL	0	NULL	biosynthetic pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The lack of reduction of the penultimate residue at the C-terminus may indicate that this step is normally at the end of the biosynthetic pathway of peptaibols and occurs with cleavage of Gly .
	manualset3
174146	8	410670	13	NULL	NULL	0	NULL	peptaibols 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The lack of reduction of the penultimate residue at the C-terminus may indicate that this step is normally at the end of the biosynthetic pathway of peptaibols and occurs with cleavage of Gly .
	manualset3
174147	9	410670	13	NULL	NULL	0	NULL	cleavage 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The lack of reduction of the penultimate residue at the C-terminus may indicate that this step is normally at the end of the biosynthetic pathway of peptaibols and occurs with cleavage of Gly .
	manualset3
174148	10	410670	13	NULL	NULL	0	NULL	Gly 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The lack of reduction of the penultimate residue at the C-terminus may indicate that this step is normally at the end of the biosynthetic pathway of peptaibols and occurs with cleavage of Gly .
	manualset3
174149	1	410671	13	NULL	NULL	0	NULL	herd 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The lacking herd immunity was partly a consequence of problems related to the vaccination system and even more of the rapid increase of the fox population .
	manualset3
174150	2	410671	13	NULL	NULL	0	NULL	immunity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The lacking herd immunity was partly a consequence of problems related to the vaccination system and even more of the rapid increase of the fox population .
	manualset3
174151	3	410671	13	NULL	NULL	0	NULL	consequence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The lacking herd immunity was partly a consequence of problems related to the vaccination system and even more of the rapid increase of the fox population .
	manualset3
174152	4	410671	13	NULL	NULL	0	NULL	problems 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The lacking herd immunity was partly a consequence of problems related to the vaccination system and even more of the rapid increase of the fox population .
	manualset3
174153	5	410671	13	NULL	NULL	0	NULL	vaccination system	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The lacking herd immunity was partly a consequence of problems related to the vaccination system and even more of the rapid increase of the fox population .
	manualset3
174154	6	410671	13	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The lacking herd immunity was partly a consequence of problems related to the vaccination system and even more of the rapid increase of the fox population .
	manualset3
174155	7	410671	13	NULL	NULL	0	NULL	fox population	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The lacking herd immunity was partly a consequence of problems related to the vaccination system and even more of the rapid increase of the fox population .
	manualset3
174156	1	410672	13	NULL	NULL	0	NULL	lag time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The lag time was not influenced by the pH value of the release medium or by the rotation speeds .
	manualset3
174157	2	410672	13	NULL	NULL	0	NULL	pH value	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The lag time was not influenced by the pH value of the release medium or by the rotation speeds .
	manualset3
174158	3	410672	13	NULL	NULL	0	NULL	release 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The lag time was not influenced by the pH value of the release medium or by the rotation speeds .
	manualset3
174159	4	410672	13	NULL	NULL	0	NULL	medium 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The lag time was not influenced by the pH value of the release medium or by the rotation speeds .
	manualset3
174160	5	410672	13	NULL	NULL	0	NULL	rotation speeds	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The lag time was not influenced by the pH value of the release medium or by the rotation speeds .
	manualset3
174161	1	410673	13	NULL	NULL	0	NULL	lamina propria	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The lamina propria did not show any labeling in either group of patients at the end of two hours .
	manualset3
174162	2	410673	13	NULL	NULL	0	NULL	labeling 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The lamina propria did not show any labeling in either group of patients at the end of two hours .
	manualset3
174163	3	410673	13	NULL	NULL	0	NULL	group of patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The lamina propria did not show any labeling in either group of patients at the end of two hours .
	manualset3
174164	4	410673	13	NULL	NULL	0	NULL	end 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The lamina propria did not show any labeling in either group of patients at the end of two hours .
	manualset3
174165	5	410673	13	NULL	NULL	0	NULL	two hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The lamina propria did not show any labeling in either group of patients at the end of two hours .
	manualset3
174166	1	410674	13	NULL	NULL	0	NULL	total 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 325 patients all older than 65 years ( 45 of more than 80 years of age ) were treated with ofloxacin during phase II studies .
	manualset3
174167	2	410674	13	NULL	NULL	0	NULL	325 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 325 patients all older than 65 years ( 45 of more than 80 years of age ) were treated with ofloxacin during phase II studies .
	manualset3
174168	3	410674	13	NULL	NULL	0	NULL	65 years	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 325 patients all older than 65 years ( 45 of more than 80 years of age ) were treated with ofloxacin during phase II studies .
	manualset3
174169	4	410674	13	NULL	NULL	0	NULL	45 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 325 patients all older than 65 years ( 45 of more than 80 years of age ) were treated with ofloxacin during phase II studies .
	manualset3
174170	5	410674	13	NULL	NULL	0	NULL	80 years of age	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 325 patients all older than 65 years ( 45 of more than 80 years of age ) were treated with ofloxacin during phase II studies .
	manualset3
174171	6	410674	13	NULL	NULL	0	NULL	ofloxacin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 325 patients all older than 65 years ( 45 of more than 80 years of age ) were treated with ofloxacin during phase II studies .
	manualset3
174172	7	410674	13	NULL	NULL	0	NULL	phase II studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 325 patients all older than 65 years ( 45 of more than 80 years of age ) were treated with ofloxacin during phase II studies .
	manualset3
174173	1	410675	13	NULL	NULL	0	NULL	language 	Language												NULL		0	NULL	NULL	NULL	NULL	NULL	The language environment of autistic and dysphasic children .
	manualset3
174174	2	410675	13	NULL	NULL	0	NULL	environment 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The language environment of autistic and dysphasic children .
	manualset3
174175	3	410675	13	NULL	NULL	0	NULL	autistic children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The language environment of autistic and dysphasic children .
	manualset3
174176	4	410675	13	NULL	NULL	0	NULL	dysphasic children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The language environment of autistic and dysphasic children .
	manualset3
174177	1	410676	13	NULL	NULL	0	NULL	large amino-terminal noncollagenous domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The large amino-terminal noncollagenous domain of type VII collagen interacts with various extracellular matrix proteins and contributes to the dermal-epidermal attachment .
	manualset3
174178	2	410676	13	NULL	NULL	0	NULL	type VII collagen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The large amino-terminal noncollagenous domain of type VII collagen interacts with various extracellular matrix proteins and contributes to the dermal-epidermal attachment .
	manualset3
174179	3	410676	13	NULL	NULL	0	NULL	extracellular matrix proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The large amino-terminal noncollagenous domain of type VII collagen interacts with various extracellular matrix proteins and contributes to the dermal-epidermal attachment .
	manualset3
174180	4	410676	13	NULL	NULL	0	NULL	dermal-epidermal attachment 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The large amino-terminal noncollagenous domain of type VII collagen interacts with various extracellular matrix proteins and contributes to the dermal-epidermal attachment .
	manualset3
174181	1	410677	13	NULL	NULL	0	NULL	ampullate glands	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The large ampullate glands of Nephila clavipes synthesize a tissue-specific fibroin for the web and dragline .
	manualset3
174182	2	410677	13	NULL	NULL	0	NULL	Nephila clavipes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The large ampullate glands of Nephila clavipes synthesize a tissue-specific fibroin for the web and dragline .
	manualset3
174183	3	410677	13	NULL	NULL	0	NULL	fibroin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The large ampullate glands of Nephila clavipes synthesize a tissue-specific fibroin for the web and dragline .
	manualset3
174184	4	410677	13	NULL	NULL	0	NULL	web 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The large ampullate glands of Nephila clavipes synthesize a tissue-specific fibroin for the web and dragline .
	manualset3
174185	1	410678	13	NULL	NULL	NULL	NULL	large group 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The large group practice survey data supported the key importance of day-to-day practice environment and relationships with patients and physician peers .
	manualset3
174186	2	410678	13	NULL	NULL	0	NULL	practice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The large group practice survey data supported the key importance of day-to-day practice environment and relationships with patients and physician peers .
	manualset3
174187	3	410678	13	NULL	NULL	0	NULL	survey data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The large group practice survey data supported the key importance of day-to-day practice environment and relationships with patients and physician peers .
	manualset3
174188	4	410678	13	NULL	NULL	0	NULL	importance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The large group practice survey data supported the key importance of day-to-day practice environment and relationships with patients and physician peers .
	manualset3
174189	5	410678	13	NULL	NULL	0	NULL	day-to-day practice 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The large group practice survey data supported the key importance of day-to-day practice environment and relationships with patients and physician peers .
	manualset3
174190	6	410678	13	NULL	NULL	0	NULL	environment 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The large group practice survey data supported the key importance of day-to-day practice environment and relationships with patients and physician peers .
	manualset3
174191	7	410678	13	NULL	NULL	0	NULL	relationships 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The large group practice survey data supported the key importance of day-to-day practice environment and relationships with patients and physician peers .
	manualset3
174192	8	410678	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The large group practice survey data supported the key importance of day-to-day practice environment and relationships with patients and physician peers .
	manualset3
174193	9	410678	13	NULL	NULL	0	NULL	physician peers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The large group practice survey data supported the key importance of day-to-day practice environment and relationships with patients and physician peers .
	manualset3
174194	1	410679	13	NULL	NULL	0	NULL	large particle	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The large particle sorting device was capable of purifying fluorescently labeled embryoid bodies ( EBs ) from unlabelled EBs with an efficiency of 87.3 % 13.5 % , and enrichment ratio of 12.28.4 ( n = 8 ) , while preserving cell viability , differentiation potential , and long-term function .
	manualset3
174195	2	410679	13	NULL	NULL	0	NULL	device 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The large particle sorting device was capable of purifying fluorescently labeled embryoid bodies ( EBs ) from unlabelled EBs with an efficiency of 87.3 % 13.5 % , and enrichment ratio of 12.28.4 ( n = 8 ) , while preserving cell viability , differentiation potential , and long-term function .
	manualset3
174196	3	410679	13	NULL	NULL	0	NULL	embryoid bodies ( EBs )	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The large particle sorting device was capable of purifying fluorescently labeled embryoid bodies ( EBs ) from unlabelled EBs with an efficiency of 87.3 % 13.5 % , and enrichment ratio of 12.28.4 ( n = 8 ) , while preserving cell viability , differentiation potential , and long-term function .
	manualset3
174197	4	410679	13	NULL	NULL	0	NULL	EBs 	cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The large particle sorting device was capable of purifying fluorescently labeled embryoid bodies ( EBs ) from unlabelled EBs with an efficiency of 87.3 % 13.5 % , and enrichment ratio of 12.28.4 ( n = 8 ) , while preserving cell viability , differentiation potential , and long-term function .
	manualset3
174198	5	410679	13	NULL	NULL	0	NULL	efficiency 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The large particle sorting device was capable of purifying fluorescently labeled embryoid bodies ( EBs ) from unlabelled EBs with an efficiency of 87.3 % 13.5 % , and enrichment ratio of 12.28.4 ( n = 8 ) , while preserving cell viability , differentiation potential , and long-term function .
	manualset3
174199	6	410679	13	NULL	NULL	0	NULL	87.3 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The large particle sorting device was capable of purifying fluorescently labeled embryoid bodies ( EBs ) from unlabelled EBs with an efficiency of 87.3 % 13.5 % , and enrichment ratio of 12.28.4 ( n = 8 ) , while preserving cell viability , differentiation potential , and long-term function .
	manualset3
174200	7	410679	13	NULL	NULL	0	NULL	13.5 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The large particle sorting device was capable of purifying fluorescently labeled embryoid bodies ( EBs ) from unlabelled EBs with an efficiency of 87.3 % 13.5 % , and enrichment ratio of 12.28.4 ( n = 8 ) , while preserving cell viability , differentiation potential , and long-term function .
	manualset3
174201	8	410679	13	NULL	NULL	0	NULL	enrichment ratio	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The large particle sorting device was capable of purifying fluorescently labeled embryoid bodies ( EBs ) from unlabelled EBs with an efficiency of 87.3 % 13.5 % , and enrichment ratio of 12.28.4 ( n = 8 ) , while preserving cell viability , differentiation potential , and long-term function .
	manualset3
174202	9	410679	13	NULL	NULL	0	NULL	12.28.4 ( n = 8 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The large particle sorting device was capable of purifying fluorescently labeled embryoid bodies ( EBs ) from unlabelled EBs with an efficiency of 87.3 % 13.5 % , and enrichment ratio of 12.28.4 ( n = 8 ) , while preserving cell viability , differentiation potential , and long-term function .
	manualset3
174203	10	410679	13	NULL	NULL	0	NULL	cell viability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The large particle sorting device was capable of purifying fluorescently labeled embryoid bodies ( EBs ) from unlabelled EBs with an efficiency of 87.3 % 13.5 % , and enrichment ratio of 12.28.4 ( n = 8 ) , while preserving cell viability , differentiation potential , and long-term function .
	manualset3
174204	11	410679	13	NULL	NULL	0	NULL	differentiation potential 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The large particle sorting device was capable of purifying fluorescently labeled embryoid bodies ( EBs ) from unlabelled EBs with an efficiency of 87.3 % 13.5 % , and enrichment ratio of 12.28.4 ( n = 8 ) , while preserving cell viability , differentiation potential , and long-term function .
	manualset3
174205	12	410679	13	NULL	NULL	0	NULL	long-term function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The large particle sorting device was capable of purifying fluorescently labeled embryoid bodies ( EBs ) from unlabelled EBs with an efficiency of 87.3 % 13.5 % , and enrichment ratio of 12.28.4 ( n = 8 ) , while preserving cell viability , differentiation potential , and long-term function .
	manualset3
174206	1	410680	13	NULL	NULL	0	NULL	size 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The large size of the serpin reactive site loop ( RSL ) suggests that the role of the RSL in protease inhibition is more complex than that of presenting the reactive site ( P1 residue ) to the protease .
	manualset3
174207	2	410680	13	NULL	NULL	0	NULL	serpin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The large size of the serpin reactive site loop ( RSL ) suggests that the role of the RSL in protease inhibition is more complex than that of presenting the reactive site ( P1 residue ) to the protease .
	manualset3
174208	3	410680	13	NULL	NULL	0	NULL	reactive site loop ( RSL )	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The large size of the serpin reactive site loop ( RSL ) suggests that the role of the RSL in protease inhibition is more complex than that of presenting the reactive site ( P1 residue ) to the protease .
	manualset3
174209	4	410680	13	NULL	NULL	0	NULL	role 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The large size of the serpin reactive site loop ( RSL ) suggests that the role of the RSL in protease inhibition is more complex than that of presenting the reactive site ( P1 residue ) to the protease .
	manualset3
174210	5	410680	13	NULL	NULL	0	NULL	RSL 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The large size of the serpin reactive site loop ( RSL ) suggests that the role of the RSL in protease inhibition is more complex than that of presenting the reactive site ( P1 residue ) to the protease .
	manualset3
174211	6	410680	13	NULL	NULL	0	NULL	protease 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The large size of the serpin reactive site loop ( RSL ) suggests that the role of the RSL in protease inhibition is more complex than that of presenting the reactive site ( P1 residue ) to the protease .
	manualset3
174212	7	410680	13	NULL	NULL	0	NULL	inhibition 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The large size of the serpin reactive site loop ( RSL ) suggests that the role of the RSL in protease inhibition is more complex than that of presenting the reactive site ( P1 residue ) to the protease .
	manualset3
174213	8	410680	13	NULL	NULL	0	NULL	reactive site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The large size of the serpin reactive site loop ( RSL ) suggests that the role of the RSL in protease inhibition is more complex than that of presenting the reactive site ( P1 residue ) to the protease .
	manualset3
174214	9	410680	13	NULL	NULL	0	NULL	P1 residue	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The large size of the serpin reactive site loop ( RSL ) suggests that the role of the RSL in protease inhibition is more complex than that of presenting the reactive site ( P1 residue ) to the protease .
	manualset3
174215	10	410680	13	NULL	NULL	0	NULL	protease 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The large size of the serpin reactive site loop ( RSL ) suggests that the role of the RSL in protease inhibition is more complex than that of presenting the reactive site ( P1 residue ) to the protease .
	manualset3
174216	1	410681	13	NULL	NULL	0	NULL	total 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 33 women on HRT ( mean age = 50.12 + / -5.2 ) and 51 nonusers ( mean age = 52.52 + / -7.8 ) fulfilled subject eligibility requirements and were included in the data analysis .
	manualset3
174217	2	410681	13	NULL	NULL	0	NULL	33 women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 33 women on HRT ( mean age = 50.12 + / -5.2 ) and 51 nonusers ( mean age = 52.52 + / -7.8 ) fulfilled subject eligibility requirements and were included in the data analysis .
	manualset3
174218	3	410681	13	NULL	NULL	0	NULL	HRT 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 33 women on HRT ( mean age = 50.12 + / -5.2 ) and 51 nonusers ( mean age = 52.52 + / -7.8 ) fulfilled subject eligibility requirements and were included in the data analysis .
	manualset3
174219	4	410681	13	NULL	NULL	0	NULL	mean age = 50.12 + / -5.2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 33 women on HRT ( mean age = 50.12 + / -5.2 ) and 51 nonusers ( mean age = 52.52 + / -7.8 ) fulfilled subject eligibility requirements and were included in the data analysis .
	manualset3
174220	5	410681	13	NULL	NULL	0	NULL	51 nonusers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 33 women on HRT ( mean age = 50.12 + / -5.2 ) and 51 nonusers ( mean age = 52.52 + / -7.8 ) fulfilled subject eligibility requirements and were included in the data analysis .
	manualset3
174221	6	410681	13	NULL	NULL	0	NULL	mean age = 52.52 + / -7.8	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 33 women on HRT ( mean age = 50.12 + / -5.2 ) and 51 nonusers ( mean age = 52.52 + / -7.8 ) fulfilled subject eligibility requirements and were included in the data analysis .
	manualset3
174222	7	410681	13	NULL	NULL	0	NULL	subject	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 33 women on HRT ( mean age = 50.12 + / -5.2 ) and 51 nonusers ( mean age = 52.52 + / -7.8 ) fulfilled subject eligibility requirements and were included in the data analysis .
	manualset3
174223	8	410681	13	NULL	NULL	NULL	NULL	eligibility 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A total of 33 women on HRT ( mean age = 50.12 + / -5.2 ) and 51 nonusers ( mean age = 52.52 + / -7.8 ) fulfilled subject eligibility requirements and were included in the data analysis .
	manualset3
174224	9	410681	13	NULL	NULL	0	NULL	requirements 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 33 women on HRT ( mean age = 50.12 + / -5.2 ) and 51 nonusers ( mean age = 52.52 + / -7.8 ) fulfilled subject eligibility requirements and were included in the data analysis .
	manualset3
174225	10	410681	13	NULL	NULL	0	NULL	data analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 33 women on HRT ( mean age = 50.12 + / -5.2 ) and 51 nonusers ( mean age = 52.52 + / -7.8 ) fulfilled subject eligibility requirements and were included in the data analysis .
	manualset3
174226	1	410682	13	NULL	NULL	0	NULL	goat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The last elder goat , which was anaemic and naturally infected with Trichostrongylus colubriformis , was still infested with the two scab mites , but was free from B. caprae .
	manualset3
174227	2	410682	13	NULL	NULL	0	NULL	Trichostrongylus colubriformis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The last elder goat , which was anaemic and naturally infected with Trichostrongylus colubriformis , was still infested with the two scab mites , but was free from B. caprae .
	manualset3
174228	3	410682	13	NULL	NULL	0	NULL	two scab mites	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The last elder goat , which was anaemic and naturally infected with Trichostrongylus colubriformis , was still infested with the two scab mites , but was free from B. caprae .
	manualset3
174229	4	410682	13	NULL	NULL	0	NULL	B. caprae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The last elder goat , which was anaemic and naturally infected with Trichostrongylus colubriformis , was still infested with the two scab mites , but was free from B. caprae .
	manualset3
174230	1	410683	13	NULL	NULL	0	NULL	latency 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The latency to an initial late positive peak , P300 , a measure of stimulus classification time , was not longer in the incongruent than the congruent condition .
	manualset3
174231	2	410683	13	NULL	NULL	0	NULL	initial late positive peak 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The latency to an initial late positive peak , P300 , a measure of stimulus classification time , was not longer in the incongruent than the congruent condition .
	manualset3
174232	3	410683	13	NULL	NULL	0	NULL	P300 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The latency to an initial late positive peak , P300 , a measure of stimulus classification time , was not longer in the incongruent than the congruent condition .
	manualset3
174233	4	410683	13	NULL	NULL	0	NULL	measure 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The latency to an initial late positive peak , P300 , a measure of stimulus classification time , was not longer in the incongruent than the congruent condition .
	manualset3
174234	5	410683	13	NULL	NULL	0	NULL	stimulus classification time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The latency to an initial late positive peak , P300 , a measure of stimulus classification time , was not longer in the incongruent than the congruent condition .
	manualset3
174235	6	410683	13	NULL	NULL	NULL	NULL	incongruent condition 	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The latency to an initial late positive peak , P300 , a measure of stimulus classification time , was not longer in the incongruent than the congruent condition .
	manualset3
174236	7	410683	13	NULL	NULL	NULL	NULL	congruent condition 	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The latency to an initial late positive peak , P300 , a measure of stimulus classification time , was not longer in the incongruent than the congruent condition .
	manualset3
174237	1	410684	13	NULL	NULL	0	NULL	lateral surface	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The lateral surface of the tube was used as negative control .
	manualset3
174238	2	410684	13	NULL	NULL	0	NULL	tube 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The lateral surface of the tube was used as negative control .
	manualset3
174239	3	410684	13	NULL	NULL	0	NULL	negative control	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The lateral surface of the tube was used as negative control .
	manualset3
174240	1	410685	13	NULL	NULL	0	NULL	processing 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The lateralized processing of affect in emotionally labile extraverts and introverts : central and autonomic effects .
	manualset3
174241	2	410685	13	NULL	NULL	0	NULL	affect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The lateralized processing of affect in emotionally labile extraverts and introverts : central and autonomic effects .
	manualset3
174242	3	410685	13	NULL	NULL	0	NULL	extraverts 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The lateralized processing of affect in emotionally labile extraverts and introverts : central and autonomic effects .
	manualset3
174243	4	410685	13	NULL	NULL	0	NULL	introverts 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The lateralized processing of affect in emotionally labile extraverts and introverts : central and autonomic effects .
	manualset3
174244	5	410685	13	NULL	NULL	0	NULL	central effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The lateralized processing of affect in emotionally labile extraverts and introverts : central and autonomic effects .
	manualset3
174245	6	410685	13	NULL	NULL	0	NULL	autonomic effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The lateralized processing of affect in emotionally labile extraverts and introverts : central and autonomic effects .
	manualset3
174246	1	410686	13	NULL	NULL	0	NULL	transcript	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter , however , appeared to produce the transcript when growing exponentially , indicating that Caco2 cultures provide an inducible system susceptible to in vitro manipulation .
	manualset3
174247	2	410686	13	NULL	NULL	0	NULL	latter 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter , however , appeared to produce the transcript when growing exponentially , indicating that Caco2 cultures provide an inducible system susceptible to in vitro manipulation .
	manualset3
174248	3	410686	13	NULL	NULL	0	NULL	Caco2 cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter , however , appeared to produce the transcript when growing exponentially , indicating that Caco2 cultures provide an inducible system susceptible to in vitro manipulation .
	manualset3
174249	4	410686	13	NULL	NULL	0	NULL	inducible system	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter , however , appeared to produce the transcript when growing exponentially , indicating that Caco2 cultures provide an inducible system susceptible to in vitro manipulation .
	manualset3
174250	5	410686	13	NULL	NULL	0	NULL	manipulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter , however , appeared to produce the transcript when growing exponentially , indicating that Caco2 cultures provide an inducible system susceptible to in vitro manipulation .
	manualset3
174251	1	410687	13	NULL	NULL	0	NULL	approach	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter approach is more popular , but so demanding of resources that it may prove impractical for cancer chemoprevention in all but a few instances .
	manualset3
174253	2	410687	13	NULL	NULL	0	NULL	resources	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter approach is more popular , but so demanding of resources that it may prove impractical for cancer chemoprevention in all but a few instances .
	manualset3
174254	3	410687	13	NULL	NULL	0	NULL	cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter approach is more popular , but so demanding of resources that it may prove impractical for cancer chemoprevention in all but a few instances .
	manualset3
174255	4	410687	13	NULL	NULL	0	NULL	chemoprevention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter approach is more popular , but so demanding of resources that it may prove impractical for cancer chemoprevention in all but a few instances .
	manualset3
174256	5	410687	13	NULL	NULL	0	NULL	instances	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter approach is more popular , but so demanding of resources that it may prove impractical for cancer chemoprevention in all but a few instances .
	manualset3
174257	1	410688	13	NULL	NULL	0	NULL	latter	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter include mucous granules of pulmonate molluscs , milk fat globules , and products of apocrine and holocrine secretion .
	manualset3
174258	2	410688	13	NULL	NULL	0	NULL	mucous granules	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter include mucous granules of pulmonate molluscs , milk fat globules , and products of apocrine and holocrine secretion .
	manualset3
174259	3	410688	13	NULL	NULL	0	NULL	pulmonate molluscs 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter include mucous granules of pulmonate molluscs , milk fat globules , and products of apocrine and holocrine secretion .
	manualset3
174260	4	410688	13	NULL	NULL	0	NULL	milk fat globules	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter include mucous granules of pulmonate molluscs , milk fat globules , and products of apocrine and holocrine secretion .
	manualset3
174261	5	410688	13	NULL	NULL	0	NULL	products	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter include mucous granules of pulmonate molluscs , milk fat globules , and products of apocrine and holocrine secretion .
	manualset3
174262	6	410688	13	NULL	NULL	0	NULL	apocrine secretion	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter include mucous granules of pulmonate molluscs , milk fat globules , and products of apocrine and holocrine secretion .
	manualset3
174263	7	410688	13	NULL	NULL	0	NULL	holocrine secretion	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter include mucous granules of pulmonate molluscs , milk fat globules , and products of apocrine and holocrine secretion .
	manualset3
174264	1	410689	13	NULL	NULL	0	NULL	latter	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter is reflected by its UV-vis spectrum exhibiting absorption bands in the visible region which are absent from that of 1W .
	manualset3
174265	2	410689	13	NULL	NULL	0	NULL	UV-vis spectrum	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter is reflected by its UV-vis spectrum exhibiting absorption bands in the visible region which are absent from that of 1W .
	manualset3
174266	3	410689	13	NULL	NULL	0	NULL	absorption bands 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter is reflected by its UV-vis spectrum exhibiting absorption bands in the visible region which are absent from that of 1W .
	manualset3
174267	4	410689	13	NULL	NULL	0	NULL	visible region	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter is reflected by its UV-vis spectrum exhibiting absorption bands in the visible region which are absent from that of 1W .
	manualset3
174268	5	410689	13	NULL	NULL	0	NULL	1W	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter is reflected by its UV-vis spectrum exhibiting absorption bands in the visible region which are absent from that of 1W .
	manualset3
174269	1	410690	13	NULL	NULL	0	NULL	latter	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter manifested in the surface electrocardiogram as premature atrial , junctional , or ventricular beats , as well as 2 AVB that mimicked Wenckebach or Mobitz II block .
	manualset3
174270	2	410690	13	NULL	NULL	0	NULL	surface electrocardiogram	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter manifested in the surface electrocardiogram as premature atrial , junctional , or ventricular beats , as well as 2 AVB that mimicked Wenckebach or Mobitz II block .
	manualset3
174271	3	410690	13	NULL	NULL	0	NULL	premature atrial beats	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter manifested in the surface electrocardiogram as premature atrial , junctional , or ventricular beats , as well as 2 AVB that mimicked Wenckebach or Mobitz II block .
	manualset3
174272	4	410690	13	NULL	NULL	0	NULL	junctional beats	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter manifested in the surface electrocardiogram as premature atrial , junctional , or ventricular beats , as well as 2 AVB that mimicked Wenckebach or Mobitz II block .
	manualset3
174273	5	410690	13	NULL	NULL	0	NULL	ventricular beats	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter manifested in the surface electrocardiogram as premature atrial , junctional , or ventricular beats , as well as 2 AVB that mimicked Wenckebach or Mobitz II block .
	manualset3
174274	6	410690	13	NULL	NULL	0	NULL	2 AVB 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter manifested in the surface electrocardiogram as premature atrial , junctional , or ventricular beats , as well as 2 AVB that mimicked Wenckebach or Mobitz II block .
	manualset3
174275	7	410690	13	NULL	NULL	0	NULL	Wenckebach block	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter manifested in the surface electrocardiogram as premature atrial , junctional , or ventricular beats , as well as 2 AVB that mimicked Wenckebach or Mobitz II block .
	manualset3
174276	8	410690	13	NULL	NULL	0	NULL	 Mobitz II block	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter manifested in the surface electrocardiogram as premature atrial , junctional , or ventricular beats , as well as 2 AVB that mimicked Wenckebach or Mobitz II block .
	manualset3
174277	1	410691	13	NULL	NULL	0	NULL	latter 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter may have a role in contraction because it provides additional free energy favoring completion of the cross-bridge power stroke .
	manualset3
174278	2	410691	13	NULL	NULL	0	NULL	role 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter may have a role in contraction because it provides additional free energy favoring completion of the cross-bridge power stroke .
	manualset3
174279	3	410691	13	NULL	NULL	0	NULL	contraction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter may have a role in contraction because it provides additional free energy favoring completion of the cross-bridge power stroke .
	manualset3
174280	4	410691	13	NULL	NULL	NULL	NULL	free energy	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The latter may have a role in contraction because it provides additional free energy favoring completion of the cross-bridge power stroke .
	manualset3
174281	5	410691	13	NULL	NULL	0	NULL	cross-bridge power stroke	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter may have a role in contraction because it provides additional free energy favoring completion of the cross-bridge power stroke .
	manualset3
174282	1	410692	13	NULL	NULL	0	NULL	left A ( 1 ) segment 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The left A ( 1 ) segment exhibited a fusiform configuration .
	manualset3
174283	2	410692	13	NULL	NULL	0	NULL	fusiform configuration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The left A ( 1 ) segment exhibited a fusiform configuration .
	manualset3
174284	1	410693	13	NULL	NULL	0	NULL	 left internal thoracic artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The left internal thoracic artery was anastomosed to LAD , and a new saphenous vein was anastomosed to the descending aorta proximally , and to the left circumflex artery distally , under a hypothermic circulatory arrest ( 9 minutes and 8 minutes for each anastomosis ) .
	manualset3
174285	2	410693	13	NULL	NULL	0	NULL	LAD	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The left internal thoracic artery was anastomosed to LAD , and a new saphenous vein was anastomosed to the descending aorta proximally , and to the left circumflex artery distally , under a hypothermic circulatory arrest ( 9 minutes and 8 minutes for each anastomosis ) .
	manualset3
174286	3	410693	13	NULL	NULL	0	NULL	new saphenous vein	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The left internal thoracic artery was anastomosed to LAD , and a new saphenous vein was anastomosed to the descending aorta proximally , and to the left circumflex artery distally , under a hypothermic circulatory arrest ( 9 minutes and 8 minutes for each anastomosis ) .
	manualset3
174287	4	410693	13	NULL	NULL	0	NULL	aorta	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The left internal thoracic artery was anastomosed to LAD , and a new saphenous vein was anastomosed to the descending aorta proximally , and to the left circumflex artery distally , under a hypothermic circulatory arrest ( 9 minutes and 8 minutes for each anastomosis ) .
	manualset3
174288	5	410693	13	NULL	NULL	0	NULL	left circumflex artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The left internal thoracic artery was anastomosed to LAD , and a new saphenous vein was anastomosed to the descending aorta proximally , and to the left circumflex artery distally , under a hypothermic circulatory arrest ( 9 minutes and 8 minutes for each anastomosis ) .
	manualset3
174289	6	410693	13	NULL	NULL	0	NULL	hypothermic circulatory arrest	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The left internal thoracic artery was anastomosed to LAD , and a new saphenous vein was anastomosed to the descending aorta proximally , and to the left circumflex artery distally , under a hypothermic circulatory arrest ( 9 minutes and 8 minutes for each anastomosis ) .
	manualset3
174290	7	410693	13	NULL	NULL	0	NULL	9 minutes	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The left internal thoracic artery was anastomosed to LAD , and a new saphenous vein was anastomosed to the descending aorta proximally , and to the left circumflex artery distally , under a hypothermic circulatory arrest ( 9 minutes and 8 minutes for each anastomosis ) .
	manualset3
174291	8	410693	13	NULL	NULL	0	NULL	8 minutes	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The left internal thoracic artery was anastomosed to LAD , and a new saphenous vein was anastomosed to the descending aorta proximally , and to the left circumflex artery distally , under a hypothermic circulatory arrest ( 9 minutes and 8 minutes for each anastomosis ) .
	manualset3
174292	9	410693	13	NULL	NULL	0	NULL	anastomosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The left internal thoracic artery was anastomosed to LAD , and a new saphenous vein was anastomosed to the descending aorta proximally , and to the left circumflex artery distally , under a hypothermic circulatory arrest ( 9 minutes and 8 minutes for each anastomosis ) .
	manualset3
174293	1	410694	13	NULL	NULL	0	NULL	left ventricle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The left ventricle of the ungulate heart : morphofunctional characteristics and muscle fiber orientation .
	manualset3
174294	2	410694	13	NULL	NULL	0	NULL	ungulate heart	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The left ventricle of the ungulate heart : morphofunctional characteristics and muscle fiber orientation .
	manualset3
174295	3	410694	13	NULL	NULL	0	NULL	morphofunctional characteristics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The left ventricle of the ungulate heart : morphofunctional characteristics and muscle fiber orientation .
	manualset3
174296	4	410694	13	NULL	NULL	0	NULL	muscle fiber orientation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The left ventricle of the ungulate heart : morphofunctional characteristics and muscle fiber orientation .
	manualset3
174297	1	410695	13	NULL	NULL	0	NULL	 length 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The length of the alkyl chain in the diaminoalkane did not influence the separation .
	manualset3
174298	2	410695	13	NULL	NULL	0	NULL	 alkyl chain	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The length of the alkyl chain in the diaminoalkane did not influence the separation .
	manualset3
174299	3	410695	13	NULL	NULL	0	NULL	diaminoalkane	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The length of the alkyl chain in the diaminoalkane did not influence the separation .
	manualset3
174300	4	410695	13	NULL	NULL	0	NULL	 separation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The length of the alkyl chain in the diaminoalkane did not influence the separation .
	manualset3
174301	1	410696	13	NULL	NULL	0	NULL	length	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The length of the curve from L1 to S2 was measured with a flexible ruler in 44 healthy subjects who were standing and sitting on both an SCC and a BMC .
	manualset3
174302	2	410696	13	NULL	NULL	0	NULL	curve	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The length of the curve from L1 to S2 was measured with a flexible ruler in 44 healthy subjects who were standing and sitting on both an SCC and a BMC .
	manualset3
174303	3	410696	13	NULL	NULL	0	NULL	L1 to S2 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The length of the curve from L1 to S2 was measured with a flexible ruler in 44 healthy subjects who were standing and sitting on both an SCC and a BMC .
	manualset3
174304	4	410696	13	NULL	NULL	0	NULL	flexible ruler	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The length of the curve from L1 to S2 was measured with a flexible ruler in 44 healthy subjects who were standing and sitting on both an SCC and a BMC .
	manualset3
174305	5	410696	13	NULL	NULL	0	NULL	44 healthy subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The length of the curve from L1 to S2 was measured with a flexible ruler in 44 healthy subjects who were standing and sitting on both an SCC and a BMC .
	manualset3
174306	6	410696	13	NULL	NULL	0	NULL	SCC 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The length of the curve from L1 to S2 was measured with a flexible ruler in 44 healthy subjects who were standing and sitting on both an SCC and a BMC .
	manualset3
174307	7	410696	13	NULL	NULL	0	NULL	BMC	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The length of the curve from L1 to S2 was measured with a flexible ruler in 44 healthy subjects who were standing and sitting on both an SCC and a BMC .
	manualset3
174308	1	410697	13	NULL	NULL	0	NULL	lengths	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The lengths and dry-tissue masses of all segments of the gastrointestinal tract tended to enlarge in response to increased dietary fiber , but only the total tract contents , contents of the small intestine , and length and dry-tissue mass of the caecum increased significantly .
	manualset3
174309	2	410697	13	NULL	NULL	0	NULL	dry-tissue masses	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The lengths and dry-tissue masses of all segments of the gastrointestinal tract tended to enlarge in response to increased dietary fiber , but only the total tract contents , contents of the small intestine , and length and dry-tissue mass of the caecum increased significantly .
	manualset3
174310	3	410697	13	NULL	NULL	0	NULL	segments	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The lengths and dry-tissue masses of all segments of the gastrointestinal tract tended to enlarge in response to increased dietary fiber , but only the total tract contents , contents of the small intestine , and length and dry-tissue mass of the caecum increased significantly .
	manualset3
174311	4	410697	13	NULL	NULL	0	NULL	gastrointestinal tract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The lengths and dry-tissue masses of all segments of the gastrointestinal tract tended to enlarge in response to increased dietary fiber , but only the total tract contents , contents of the small intestine , and length and dry-tissue mass of the caecum increased significantly .
	manualset3
174312	5	410697	13	NULL	NULL	0	NULL	response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The lengths and dry-tissue masses of all segments of the gastrointestinal tract tended to enlarge in response to increased dietary fiber , but only the total tract contents , contents of the small intestine , and length and dry-tissue mass of the caecum increased significantly .
	manualset3
174313	6	410697	13	NULL	NULL	0	NULL	dietary fiber	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The lengths and dry-tissue masses of all segments of the gastrointestinal tract tended to enlarge in response to increased dietary fiber , but only the total tract contents , contents of the small intestine , and length and dry-tissue mass of the caecum increased significantly .
	manualset3
174314	7	410697	13	NULL	NULL	0	NULL	total tract contents	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The lengths and dry-tissue masses of all segments of the gastrointestinal tract tended to enlarge in response to increased dietary fiber , but only the total tract contents , contents of the small intestine , and length and dry-tissue mass of the caecum increased significantly .
	manualset3
174315	8	410697	13	NULL	NULL	0	NULL	contents 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The lengths and dry-tissue masses of all segments of the gastrointestinal tract tended to enlarge in response to increased dietary fiber , but only the total tract contents , contents of the small intestine , and length and dry-tissue mass of the caecum increased significantly .
	manualset3
174316	9	410697	13	NULL	NULL	0	NULL	small intestine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The lengths and dry-tissue masses of all segments of the gastrointestinal tract tended to enlarge in response to increased dietary fiber , but only the total tract contents , contents of the small intestine , and length and dry-tissue mass of the caecum increased significantly .
	manualset3
174317	10	410697	13	NULL	NULL	0	NULL	length 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The lengths and dry-tissue masses of all segments of the gastrointestinal tract tended to enlarge in response to increased dietary fiber , but only the total tract contents , contents of the small intestine , and length and dry-tissue mass of the caecum increased significantly .
	manualset3
174318	11	410697	13	NULL	NULL	0	NULL	dry-tissue mass	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The lengths and dry-tissue masses of all segments of the gastrointestinal tract tended to enlarge in response to increased dietary fiber , but only the total tract contents , contents of the small intestine , and length and dry-tissue mass of the caecum increased significantly .
	manualset3
174319	12	410697	13	NULL	NULL	0	NULL	caecum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The lengths and dry-tissue masses of all segments of the gastrointestinal tract tended to enlarge in response to increased dietary fiber , but only the total tract contents , contents of the small intestine , and length and dry-tissue mass of the caecum increased significantly .
	manualset3
174320	1	410698	13	NULL	NULL	0	NULL	lengths	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The lengths of the deduced sequences of these transcripts were variable ( between 107 to 112 amino acids ) .
	manualset3
174321	2	410698	13	NULL	NULL	0	NULL	sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The lengths of the deduced sequences of these transcripts were variable ( between 107 to 112 amino acids ) .
	manualset3
174322	3	410698	13	NULL	NULL	0	NULL	transcripts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The lengths of the deduced sequences of these transcripts were variable ( between 107 to 112 amino acids ) .
	manualset3
174323	4	410698	13	NULL	NULL	0	NULL	107 to 112 amino acids	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The lengths of the deduced sequences of these transcripts were variable ( between 107 to 112 amino acids ) .
	manualset3
174324	1	410699	13	NULL	NULL	0	NULL	leptin receptor ( LEPR ) 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The leptin receptor ( LEPR ) is a key gene in the control of food intake and energy homeostasis .
	manualset3
174325	2	410699	13	NULL	NULL	0	NULL	gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The leptin receptor ( LEPR ) is a key gene in the control of food intake and energy homeostasis .
	manualset3
174326	3	410699	13	NULL	NULL	0	NULL	food intake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The leptin receptor ( LEPR ) is a key gene in the control of food intake and energy homeostasis .
	manualset3
174327	4	410699	13	NULL	NULL	0	NULL	energy homeostasis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The leptin receptor ( LEPR ) is a key gene in the control of food intake and energy homeostasis .
	manualset3
178672	5	410699	13	NULL	NULL	0	NULL	control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The leptin receptor ( LEPR ) is a key gene in the control of food intake and energy homeostasis .
	manualset3
174328	1	410700	13	NULL	NULL	0	NULL	leptomeningeal involvement 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The leptomeningeal involvement of central nervous system is defined in the most centers by the presence of blast cells in the CSF or the presence of cranial-nerve palsies .
	manualset3
174329	2	410700	13	NULL	NULL	0	NULL	central nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The leptomeningeal involvement of central nervous system is defined in the most centers by the presence of blast cells in the CSF or the presence of cranial-nerve palsies .
	manualset3
174330	3	410700	13	NULL	NULL	0	NULL	centers	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The leptomeningeal involvement of central nervous system is defined in the most centers by the presence of blast cells in the CSF or the presence of cranial-nerve palsies .
	manualset3
174331	4	410700	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The leptomeningeal involvement of central nervous system is defined in the most centers by the presence of blast cells in the CSF or the presence of cranial-nerve palsies .
	manualset3
174332	5	410700	13	NULL	NULL	0	NULL	blast cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The leptomeningeal involvement of central nervous system is defined in the most centers by the presence of blast cells in the CSF or the presence of cranial-nerve palsies .
	manualset3
174333	6	410700	13	NULL	NULL	0	NULL	CSF 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The leptomeningeal involvement of central nervous system is defined in the most centers by the presence of blast cells in the CSF or the presence of cranial-nerve palsies .
	manualset3
174334	7	410700	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The leptomeningeal involvement of central nervous system is defined in the most centers by the presence of blast cells in the CSF or the presence of cranial-nerve palsies .
	manualset3
174335	8	410700	13	NULL	NULL	0	NULL	cranial-nerve palsies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The leptomeningeal involvement of central nervous system is defined in the most centers by the presence of blast cells in the CSF or the presence of cranial-nerve palsies .
	manualset3
174336	1	410701	13	NULL	NULL	0	NULL	lesion area 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The lesion area after 4 hr of stress during the dark phase was significantly lower than in light-phase controls .
	manualset3
174337	2	410701	13	NULL	NULL	0	NULL	4 hr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The lesion area after 4 hr of stress during the dark phase was significantly lower than in light-phase controls .
	manualset3
174338	3	410701	13	NULL	NULL	0	NULL	stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The lesion area after 4 hr of stress during the dark phase was significantly lower than in light-phase controls .
	manualset3
174339	4	410701	13	NULL	NULL	0	NULL	dark phase	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The lesion area after 4 hr of stress during the dark phase was significantly lower than in light-phase controls .
	manualset3
174340	5	410701	13	NULL	NULL	0	NULL	light-phase controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The lesion area after 4 hr of stress during the dark phase was significantly lower than in light-phase controls .
	manualset3
174341	1	410702	13	NULL	NULL	0	NULL	lesion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The lesion covered the upper two-thirds of the right trigeminal nerve dermatome , involving half of the face with the forehead , the periorbital area , upper part of the cheek and the nose .
	manualset3
174342	2	410702	13	NULL	NULL	0	NULL	upper two-thirds 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The lesion covered the upper two-thirds of the right trigeminal nerve dermatome , involving half of the face with the forehead , the periorbital area , upper part of the cheek and the nose .
	manualset3
174343	3	410702	13	NULL	NULL	0	NULL	right trigeminal nerve dermatome	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The lesion covered the upper two-thirds of the right trigeminal nerve dermatome , involving half of the face with the forehead , the periorbital area , upper part of the cheek and the nose .
	manualset3
174344	4	410702	13	NULL	NULL	0	NULL	half 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The lesion covered the upper two-thirds of the right trigeminal nerve dermatome , involving half of the face with the forehead , the periorbital area , upper part of the cheek and the nose .
	manualset3
174345	5	410702	13	NULL	NULL	0	NULL	face	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The lesion covered the upper two-thirds of the right trigeminal nerve dermatome , involving half of the face with the forehead , the periorbital area , upper part of the cheek and the nose .
	manualset3
174346	6	410702	13	NULL	NULL	0	NULL	forehead 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The lesion covered the upper two-thirds of the right trigeminal nerve dermatome , involving half of the face with the forehead , the periorbital area , upper part of the cheek and the nose .
	manualset3
174347	7	410702	13	NULL	NULL	0	NULL	periorbital area	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The lesion covered the upper two-thirds of the right trigeminal nerve dermatome , involving half of the face with the forehead , the periorbital area , upper part of the cheek and the nose .
	manualset3
174348	8	410702	13	NULL	NULL	0	NULL	upper part	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The lesion covered the upper two-thirds of the right trigeminal nerve dermatome , involving half of the face with the forehead , the periorbital area , upper part of the cheek and the nose .
	manualset3
174349	9	410702	13	NULL	NULL	0	NULL	 cheek	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The lesion covered the upper two-thirds of the right trigeminal nerve dermatome , involving half of the face with the forehead , the periorbital area , upper part of the cheek and the nose .
	manualset3
174350	10	410702	13	NULL	NULL	0	NULL	nose	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The lesion covered the upper two-thirds of the right trigeminal nerve dermatome , involving half of the face with the forehead , the periorbital area , upper part of the cheek and the nose .
	manualset3
174351	1	410703	13	NULL	NULL	0	NULL	lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The lesion failed to respond to nafcillin alone or combination therapy with hyperbaric oxygen , but showed slow , steady improvement with long-term clindamycin .
	manualset3
174352	2	410703	13	NULL	NULL	0	NULL	nafcillin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The lesion failed to respond to nafcillin alone or combination therapy with hyperbaric oxygen , but showed slow , steady improvement with long-term clindamycin .
	manualset3
174353	3	410703	13	NULL	NULL	0	NULL	combination therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The lesion failed to respond to nafcillin alone or combination therapy with hyperbaric oxygen , but showed slow , steady improvement with long-term clindamycin .
	manualset3
174354	4	410703	13	NULL	NULL	0	NULL	hyperbaric oxygen	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The lesion failed to respond to nafcillin alone or combination therapy with hyperbaric oxygen , but showed slow , steady improvement with long-term clindamycin .
	manualset3
174355	5	410703	13	NULL	NULL	0	NULL	improvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The lesion failed to respond to nafcillin alone or combination therapy with hyperbaric oxygen , but showed slow , steady improvement with long-term clindamycin .
	manualset3
174356	6	410703	13	NULL	NULL	0	NULL	clindamycin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The lesion failed to respond to nafcillin alone or combination therapy with hyperbaric oxygen , but showed slow , steady improvement with long-term clindamycin .
	manualset3
174357	1	410704	13	NULL	NULL	0	NULL	lessons	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The lessons learned will be useful in initiating new programs and building sustainability frameworks for FETPs and FELTPs in Africa .
	manualset3
174358	2	410704	13	NULL	NULL	0	NULL	new programs	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The lessons learned will be useful in initiating new programs and building sustainability frameworks for FETPs and FELTPs in Africa .
	manualset3
174359	3	410704	13	NULL	NULL	0	NULL	building	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The lessons learned will be useful in initiating new programs and building sustainability frameworks for FETPs and FELTPs in Africa .
	manualset3
174360	4	410704	13	NULL	NULL	0	NULL	sustainability frameworks	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The lessons learned will be useful in initiating new programs and building sustainability frameworks for FETPs and FELTPs in Africa .
	manualset3
174361	5	410704	13	NULL	NULL	0	NULL	FETPs	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The lessons learned will be useful in initiating new programs and building sustainability frameworks for FETPs and FELTPs in Africa .
	manualset3
174362	6	410704	13	NULL	NULL	0	NULL	 FELTPs	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The lessons learned will be useful in initiating new programs and building sustainability frameworks for FETPs and FELTPs in Africa .
	manualset3
174363	7	410704	13	NULL	NULL	0	NULL	Africa	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The lessons learned will be useful in initiating new programs and building sustainability frameworks for FETPs and FELTPs in Africa .
	manualset3
174364	1	410705	13	NULL	NULL	0	NULL	 leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The leukemia is strain-specific and causes the death of its recipients within 9 days .
	manualset3
174365	2	410705	13	NULL	NULL	0	NULL	death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The leukemia is strain-specific and causes the death of its recipients within 9 days .
	manualset3
174366	3	410705	13	NULL	NULL	0	NULL	recipients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The leukemia is strain-specific and causes the death of its recipients within 9 days .
	manualset3
174367	4	410705	13	NULL	NULL	0	NULL	 9 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The leukemia is strain-specific and causes the death of its recipients within 9 days .
	manualset3
174368	1	410706	13	NULL	NULL	0	NULL	level 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of DcCB1 mRNAs was high in somatic embryos at globular and heart-shaped stages but low in torpedo-shaped somatic embryos .
	manualset3
174369	2	410706	13	NULL	NULL	0	NULL	 DcCB1 mRNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of DcCB1 mRNAs was high in somatic embryos at globular and heart-shaped stages but low in torpedo-shaped somatic embryos .
	manualset3
174370	3	410706	13	NULL	NULL	NULL	NULL	somatic embryos 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The level of DcCB1 mRNAs was high in somatic embryos at globular and heart-shaped stages but low in torpedo-shaped somatic embryos .
	manualset3
174371	4	410706	13	NULL	NULL	0	NULL	globular stage	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of DcCB1 mRNAs was high in somatic embryos at globular and heart-shaped stages but low in torpedo-shaped somatic embryos .
	manualset3
174372	5	410706	13	NULL	NULL	0	NULL	heart-shaped stage	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of DcCB1 mRNAs was high in somatic embryos at globular and heart-shaped stages but low in torpedo-shaped somatic embryos .
	manualset3
174373	6	410706	13	NULL	NULL	NULL	NULL	torpedo-shaped somatic embryos 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The level of DcCB1 mRNAs was high in somatic embryos at globular and heart-shaped stages but low in torpedo-shaped somatic embryos .
	manualset3
174374	1	410707	13	NULL	NULL	0	NULL	level	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of F antigen on LNC of MRL/1 , but not on those of MRL/n mice , increased progressively with age and reached its maximum at 4 mo of age .
	manualset3
174375	2	410707	13	NULL	NULL	0	NULL	F antigen	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of F antigen on LNC of MRL/1 , but not on those of MRL/n mice , increased progressively with age and reached its maximum at 4 mo of age .
	manualset3
174376	3	410707	13	NULL	NULL	0	NULL	LNC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of F antigen on LNC of MRL/1 , but not on those of MRL/n mice , increased progressively with age and reached its maximum at 4 mo of age .
	manualset3
174377	4	410707	13	NULL	NULL	0	NULL	MRL/1 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of F antigen on LNC of MRL/1 , but not on those of MRL/n mice , increased progressively with age and reached its maximum at 4 mo of age .
	manualset3
174378	5	410707	13	NULL	NULL	0	NULL	MRL/n mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of F antigen on LNC of MRL/1 , but not on those of MRL/n mice , increased progressively with age and reached its maximum at 4 mo of age .
	manualset3
174379	6	410707	13	NULL	NULL	0	NULL	age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of F antigen on LNC of MRL/1 , but not on those of MRL/n mice , increased progressively with age and reached its maximum at 4 mo of age .
	manualset3
174380	7	410707	13	NULL	NULL	0	NULL	4 mo of age	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of F antigen on LNC of MRL/1 , but not on those of MRL/n mice , increased progressively with age and reached its maximum at 4 mo of age .
	manualset3
178673	8	410707	13	NULL	NULL	0	NULL	maximum 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of F antigen on LNC of MRL/1 , but not on those of MRL/n mice , increased progressively with age and reached its maximum at 4 mo of age .
	manualset3
174381	1	410708	13	NULL	NULL	0	NULL	 level	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of NO produced by inhibitory concentrations of SNAP was comparable to NO levels produced by the induction of inducible nitric oxide synthase ( iNOS ) in smooth muscle cells or retinal pigmented epithelial cells .
	manualset3
174382	2	410708	13	NULL	NULL	0	NULL	NO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of NO produced by inhibitory concentrations of SNAP was comparable to NO levels produced by the induction of inducible nitric oxide synthase ( iNOS ) in smooth muscle cells or retinal pigmented epithelial cells .
	manualset3
174383	3	410708	13	NULL	NULL	0	NULL	concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of NO produced by inhibitory concentrations of SNAP was comparable to NO levels produced by the induction of inducible nitric oxide synthase ( iNOS ) in smooth muscle cells or retinal pigmented epithelial cells .
	manualset3
174384	4	410708	13	NULL	NULL	0	NULL	SNAP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of NO produced by inhibitory concentrations of SNAP was comparable to NO levels produced by the induction of inducible nitric oxide synthase ( iNOS ) in smooth muscle cells or retinal pigmented epithelial cells .
	manualset3
174385	5	410708	13	NULL	NULL	0	NULL	NO levels 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of NO produced by inhibitory concentrations of SNAP was comparable to NO levels produced by the induction of inducible nitric oxide synthase ( iNOS ) in smooth muscle cells or retinal pigmented epithelial cells .
	manualset3
174386	6	410708	13	NULL	NULL	0	NULL	induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of NO produced by inhibitory concentrations of SNAP was comparable to NO levels produced by the induction of inducible nitric oxide synthase ( iNOS ) in smooth muscle cells or retinal pigmented epithelial cells .
	manualset3
174387	7	410708	13	NULL	NULL	0	NULL	inducible nitric oxide synthase ( iNOS ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of NO produced by inhibitory concentrations of SNAP was comparable to NO levels produced by the induction of inducible nitric oxide synthase ( iNOS ) in smooth muscle cells or retinal pigmented epithelial cells .
	manualset3
174388	8	410708	13	NULL	NULL	0	NULL	smooth muscle cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of NO produced by inhibitory concentrations of SNAP was comparable to NO levels produced by the induction of inducible nitric oxide synthase ( iNOS ) in smooth muscle cells or retinal pigmented epithelial cells .
	manualset3
174389	9	410708	13	NULL	NULL	0	NULL	retinal pigmented epithelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of NO produced by inhibitory concentrations of SNAP was comparable to NO levels produced by the induction of inducible nitric oxide synthase ( iNOS ) in smooth muscle cells or retinal pigmented epithelial cells .
	manualset3
174390	1	410709	13	NULL	NULL	0	NULL	level	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of c-Myc and D-cyclins , proteins involved in p27KiP1 sequestration , decreased in the absence of functional ErbB2 .
	manualset3
174391	2	410709	13	NULL	NULL	0	NULL	c-Myc	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of c-Myc and D-cyclins , proteins involved in p27KiP1 sequestration , decreased in the absence of functional ErbB2 .
	manualset3
174392	3	410709	13	NULL	NULL	NULL	NULL	D-cyclins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The level of c-Myc and D-cyclins , proteins involved in p27KiP1 sequestration , decreased in the absence of functional ErbB2 .
	manualset3
174393	4	410709	13	NULL	NULL	0	NULL	proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of c-Myc and D-cyclins , proteins involved in p27KiP1 sequestration , decreased in the absence of functional ErbB2 .
	manualset3
174394	5	410709	13	NULL	NULL	0	NULL	p27KiP1 sequestration	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of c-Myc and D-cyclins , proteins involved in p27KiP1 sequestration , decreased in the absence of functional ErbB2 .
	manualset3
174395	6	410709	13	NULL	NULL	0	NULL	 absence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of c-Myc and D-cyclins , proteins involved in p27KiP1 sequestration , decreased in the absence of functional ErbB2 .
	manualset3
174396	7	410709	13	NULL	NULL	0	NULL	ErbB2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of c-Myc and D-cyclins , proteins involved in p27KiP1 sequestration , decreased in the absence of functional ErbB2 .
	manualset3
174397	1	410710	13	NULL	NULL	0	NULL	level	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of connexin43 mRNA is maximally upregulated 48 h after treatment with recombinant human BMP-2 with corresponding changes in protein expression .
	manualset3
174398	2	410710	13	NULL	NULL	0	NULL	connexin43 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of connexin43 mRNA is maximally upregulated 48 h after treatment with recombinant human BMP-2 with corresponding changes in protein expression .
	manualset3
174399	3	410710	13	NULL	NULL	0	NULL	48 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of connexin43 mRNA is maximally upregulated 48 h after treatment with recombinant human BMP-2 with corresponding changes in protein expression .
	manualset3
174400	4	410710	13	NULL	NULL	0	NULL	treatment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of connexin43 mRNA is maximally upregulated 48 h after treatment with recombinant human BMP-2 with corresponding changes in protein expression .
	manualset3
174401	5	410710	13	NULL	NULL	0	NULL	recombinant human BMP-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of connexin43 mRNA is maximally upregulated 48 h after treatment with recombinant human BMP-2 with corresponding changes in protein expression .
	manualset3
174402	6	410710	13	NULL	NULL	0	NULL	changes 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of connexin43 mRNA is maximally upregulated 48 h after treatment with recombinant human BMP-2 with corresponding changes in protein expression .
	manualset3
174403	7	410710	13	NULL	NULL	0	NULL	protein expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of connexin43 mRNA is maximally upregulated 48 h after treatment with recombinant human BMP-2 with corresponding changes in protein expression .
	manualset3
174404	1	410711	13	NULL	NULL	0	NULL	 level 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of education is related to exposure to media as well as the use of family planning methods , and negatively related to the degree of apprehension .
	manualset3
174405	2	410711	13	NULL	NULL	0	NULL	education	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of education is related to exposure to media as well as the use of family planning methods , and negatively related to the degree of apprehension .
	manualset3
174406	3	410711	13	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of education is related to exposure to media as well as the use of family planning methods , and negatively related to the degree of apprehension .
	manualset3
174407	4	410711	13	NULL	NULL	0	NULL	media	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of education is related to exposure to media as well as the use of family planning methods , and negatively related to the degree of apprehension .
	manualset3
174408	5	410711	13	NULL	NULL	0	NULL	family planning methods	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of education is related to exposure to media as well as the use of family planning methods , and negatively related to the degree of apprehension .
	manualset3
174409	6	410711	13	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of education is related to exposure to media as well as the use of family planning methods , and negatively related to the degree of apprehension .
	manualset3
174410	7	410711	13	NULL	NULL	0	NULL	degree	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of education is related to exposure to media as well as the use of family planning methods , and negatively related to the degree of apprehension .
	manualset3
174411	8	410711	13	NULL	NULL	0	NULL	apprehension	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of education is related to exposure to media as well as the use of family planning methods , and negatively related to the degree of apprehension .
	manualset3
174412	1	410712	13	NULL	NULL	0	NULL	 level of infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of infection by infectious pancreatic necrosis virus ( IPNV ) of kidney macrophages from 12 asymptomatic carrier Atlantic salmon post-smolts was studied .
	manualset3
174413	2	410712	13	NULL	NULL	0	NULL	infectious pancreatic necrosis virus ( IPNV ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of infection by infectious pancreatic necrosis virus ( IPNV ) of kidney macrophages from 12 asymptomatic carrier Atlantic salmon post-smolts was studied .
	manualset3
174414	3	410712	13	NULL	NULL	0	NULL	kidney macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of infection by infectious pancreatic necrosis virus ( IPNV ) of kidney macrophages from 12 asymptomatic carrier Atlantic salmon post-smolts was studied .
	manualset3
174415	4	410712	13	NULL	NULL	0	NULL	12 asymptomatic carrier Atlantic salmon post-smolts	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of infection by infectious pancreatic necrosis virus ( IPNV ) of kidney macrophages from 12 asymptomatic carrier Atlantic salmon post-smolts was studied .
	manualset3
174416	1	410713	13	NULL	NULL	0	NULL	 level	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of major pathogen infection in cows completing the trial in all herds increased in the partial treatment group from 5 per cent of quarters at the start to 12 per cent at the finish of the trial .
	manualset3
174417	2	410713	13	NULL	NULL	0	NULL	major pathogen infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of major pathogen infection in cows completing the trial in all herds increased in the partial treatment group from 5 per cent of quarters at the start to 12 per cent at the finish of the trial .
	manualset3
174418	3	410713	13	NULL	NULL	0	NULL	 cows	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of major pathogen infection in cows completing the trial in all herds increased in the partial treatment group from 5 per cent of quarters at the start to 12 per cent at the finish of the trial .
	manualset3
174419	4	410713	13	NULL	NULL	0	NULL	trial	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of major pathogen infection in cows completing the trial in all herds increased in the partial treatment group from 5 per cent of quarters at the start to 12 per cent at the finish of the trial .
	manualset3
174420	5	410713	13	NULL	NULL	0	NULL	herds	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of major pathogen infection in cows completing the trial in all herds increased in the partial treatment group from 5 per cent of quarters at the start to 12 per cent at the finish of the trial .
	manualset3
174421	6	410713	13	NULL	NULL	0	NULL	partial treatment group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of major pathogen infection in cows completing the trial in all herds increased in the partial treatment group from 5 per cent of quarters at the start to 12 per cent at the finish of the trial .
	manualset3
174422	7	410713	13	NULL	NULL	0	NULL	5 per cent of quarters	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of major pathogen infection in cows completing the trial in all herds increased in the partial treatment group from 5 per cent of quarters at the start to 12 per cent at the finish of the trial .
	manualset3
174423	8	410713	13	NULL	NULL	0	NULL	start	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of major pathogen infection in cows completing the trial in all herds increased in the partial treatment group from 5 per cent of quarters at the start to 12 per cent at the finish of the trial .
	manualset3
174424	9	410713	13	NULL	NULL	0	NULL	12 per cent 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of major pathogen infection in cows completing the trial in all herds increased in the partial treatment group from 5 per cent of quarters at the start to 12 per cent at the finish of the trial .
	manualset3
174425	10	410713	13	NULL	NULL	0	NULL	finish 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of major pathogen infection in cows completing the trial in all herds increased in the partial treatment group from 5 per cent of quarters at the start to 12 per cent at the finish of the trial .
	manualset3
174426	11	410713	13	NULL	NULL	0	NULL	trial	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of major pathogen infection in cows completing the trial in all herds increased in the partial treatment group from 5 per cent of quarters at the start to 12 per cent at the finish of the trial .
	manualset3
174427	1	410714	13	NULL	NULL	0	NULL	level 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of modification of H2 was , however , presumably an exception , as it was significantly lower for both larvae and adults in D. virilis than in the other two species .
	manualset3
174428	2	410714	13	NULL	NULL	0	NULL	modification	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of modification of H2 was , however , presumably an exception , as it was significantly lower for both larvae and adults in D. virilis than in the other two species .
	manualset3
174429	3	410714	13	NULL	NULL	0	NULL	 H2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of modification of H2 was , however , presumably an exception , as it was significantly lower for both larvae and adults in D. virilis than in the other two species .
	manualset3
174430	4	410714	13	NULL	NULL	0	NULL	exception	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of modification of H2 was , however , presumably an exception , as it was significantly lower for both larvae and adults in D. virilis than in the other two species .
	manualset3
174431	5	410714	13	NULL	NULL	0	NULL	larvae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of modification of H2 was , however , presumably an exception , as it was significantly lower for both larvae and adults in D. virilis than in the other two species .
	manualset3
174432	6	410714	13	NULL	NULL	0	NULL	adults	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of modification of H2 was , however , presumably an exception , as it was significantly lower for both larvae and adults in D. virilis than in the other two species .
	manualset3
174433	7	410714	13	NULL	NULL	0	NULL	D. virilis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of modification of H2 was , however , presumably an exception , as it was significantly lower for both larvae and adults in D. virilis than in the other two species .
	manualset3
174434	8	410714	13	NULL	NULL	0	NULL	 two species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of modification of H2 was , however , presumably an exception , as it was significantly lower for both larvae and adults in D. virilis than in the other two species .
	manualset3
174435	1	410715	13	NULL	NULL	0	NULL	total 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 49 patients with chronic ischaemic heart disease ( 38 of whom had previously survived myoca dial infarction ) were treated with Piridoxylate administered intramuscularly and orally .
	manualset3
174436	2	410715	13	NULL	NULL	0	NULL	49 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 49 patients with chronic ischaemic heart disease ( 38 of whom had previously survived myoca dial infarction ) were treated with Piridoxylate administered intramuscularly and orally .
	manualset3
174437	3	410715	13	NULL	NULL	0	NULL	chronic ischaemic heart disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 49 patients with chronic ischaemic heart disease ( 38 of whom had previously survived myoca dial infarction ) were treated with Piridoxylate administered intramuscularly and orally .
	manualset3
174438	4	410715	13	NULL	NULL	0	NULL	 38	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 49 patients with chronic ischaemic heart disease ( 38 of whom had previously survived myoca dial infarction ) were treated with Piridoxylate administered intramuscularly and orally .
	manualset3
174439	5	410715	13	NULL	NULL	0	NULL	myoca dial infarction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 49 patients with chronic ischaemic heart disease ( 38 of whom had previously survived myoca dial infarction ) were treated with Piridoxylate administered intramuscularly and orally .
	manualset3
174440	6	410715	13	NULL	NULL	0	NULL	Piridoxylate	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 49 patients with chronic ischaemic heart disease ( 38 of whom had previously survived myoca dial infarction ) were treated with Piridoxylate administered intramuscularly and orally .
	manualset3
174441	1	410716	13	NULL	NULL	0	NULL	level of radioactivity 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of radioactivity from the quadriceps femoris was determined before exercise and during two periods post-exercise .
	manualset3
174442	2	410716	13	NULL	NULL	0	NULL	quadriceps femoris 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of radioactivity from the quadriceps femoris was determined before exercise and during two periods post-exercise .
	manualset3
174443	3	410716	13	NULL	NULL	0	NULL	exercise 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of radioactivity from the quadriceps femoris was determined before exercise and during two periods post-exercise .
	manualset3
174444	4	410716	13	NULL	NULL	0	NULL	two periods	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of radioactivity from the quadriceps femoris was determined before exercise and during two periods post-exercise .
	manualset3
174445	5	410716	13	NULL	NULL	0	NULL	post-exercise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of radioactivity from the quadriceps femoris was determined before exercise and during two periods post-exercise .
	manualset3
174446	1	410717	13	NULL	NULL	0	NULL	level	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of undercarboxylated osteocalcin is recognized as a marker of vitamin K2 bone .
	manualset3
174447	2	410717	13	NULL	NULL	0	NULL	undercarboxylated osteocalcin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of undercarboxylated osteocalcin is recognized as a marker of vitamin K2 bone .
	manualset3
174449	4	410717	13	NULL	NULL	0	NULL	vitamin K2 bone	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of undercarboxylated osteocalcin is recognized as a marker of vitamin K2 bone .
	manualset3
178674	5	410717	13	NULL	NULL	0	NULL	marker	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The level of undercarboxylated osteocalcin is recognized as a marker of vitamin K2 bone .
	manualset3
174448	1	410718	13	NULL	NULL	NULL	NULL	levels	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The levels detected ranged from 0.09 to 2.34 micro g/g of dust .
	manualset3
174450	2	410718	13	NULL	NULL	0	NULL	0.09 to 2.34 micro g/g of dust	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels detected ranged from 0.09 to 2.34 micro g/g of dust .
	manualset3
174451	1	410719	13	NULL	NULL	0	NULL	levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of asymmetric induction were influenced by solvent polarity , acid strength and , to a lesser extent , temperature .
	manualset3
174452	2	410719	13	NULL	NULL	0	NULL	asymmetric induction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of asymmetric induction were influenced by solvent polarity , acid strength and , to a lesser extent , temperature .
	manualset3
174453	3	410719	13	NULL	NULL	0	NULL	solvent polarity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of asymmetric induction were influenced by solvent polarity , acid strength and , to a lesser extent , temperature .
	manualset3
174454	4	410719	13	NULL	NULL	0	NULL	acid strength	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of asymmetric induction were influenced by solvent polarity , acid strength and , to a lesser extent , temperature .
	manualset3
174455	5	410719	13	NULL	NULL	0	NULL	temperature	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of asymmetric induction were influenced by solvent polarity , acid strength and , to a lesser extent , temperature .
	manualset3
174456	1	410720	13	NULL	NULL	0	NULL	levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of cellular retinol-binding protein ( CRBP ) and cellular retinoic acid-binding protein ( CRABP ) were determined in 37 squamous cell carcinomas of the head and neck and were compared with the corresponding levels in adjacent normal tissue .
	manualset3
174457	2	410720	13	NULL	NULL	0	NULL	cellular retinol-binding protein ( CRBP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of cellular retinol-binding protein ( CRBP ) and cellular retinoic acid-binding protein ( CRABP ) were determined in 37 squamous cell carcinomas of the head and neck and were compared with the corresponding levels in adjacent normal tissue .
	manualset3
174458	3	410720	13	NULL	NULL	0	NULL	 cellular retinoic acid-binding protein ( CRABP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of cellular retinol-binding protein ( CRBP ) and cellular retinoic acid-binding protein ( CRABP ) were determined in 37 squamous cell carcinomas of the head and neck and were compared with the corresponding levels in adjacent normal tissue .
	manualset3
174459	4	410720	13	NULL	NULL	0	NULL	37 squamous cell carcinomas	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of cellular retinol-binding protein ( CRBP ) and cellular retinoic acid-binding protein ( CRABP ) were determined in 37 squamous cell carcinomas of the head and neck and were compared with the corresponding levels in adjacent normal tissue .
	manualset3
174460	5	410720	13	NULL	NULL	0	NULL	head 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of cellular retinol-binding protein ( CRBP ) and cellular retinoic acid-binding protein ( CRABP ) were determined in 37 squamous cell carcinomas of the head and neck and were compared with the corresponding levels in adjacent normal tissue .
	manualset3
174461	6	410720	13	NULL	NULL	0	NULL	neck 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of cellular retinol-binding protein ( CRBP ) and cellular retinoic acid-binding protein ( CRABP ) were determined in 37 squamous cell carcinomas of the head and neck and were compared with the corresponding levels in adjacent normal tissue .
	manualset3
174462	7	410720	13	NULL	NULL	0	NULL	levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of cellular retinol-binding protein ( CRBP ) and cellular retinoic acid-binding protein ( CRABP ) were determined in 37 squamous cell carcinomas of the head and neck and were compared with the corresponding levels in adjacent normal tissue .
	manualset3
174463	8	410720	13	NULL	NULL	0	NULL	tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of cellular retinol-binding protein ( CRBP ) and cellular retinoic acid-binding protein ( CRABP ) were determined in 37 squamous cell carcinomas of the head and neck and were compared with the corresponding levels in adjacent normal tissue .
	manualset3
174464	1	410721	13	NULL	NULL	0	NULL	levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of lipid peroxidation and the activity of catalase , glutathione peroxidase ( GPx ) , glutathione S-transferase ( GST ) and glutathione reductase ( GR ) were carried out in brain homogenates of SNP-injected mice .
	manualset3
174465	2	410721	13	NULL	NULL	0	NULL	lipid peroxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of lipid peroxidation and the activity of catalase , glutathione peroxidase ( GPx ) , glutathione S-transferase ( GST ) and glutathione reductase ( GR ) were carried out in brain homogenates of SNP-injected mice .
	manualset3
174466	3	410721	13	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of lipid peroxidation and the activity of catalase , glutathione peroxidase ( GPx ) , glutathione S-transferase ( GST ) and glutathione reductase ( GR ) were carried out in brain homogenates of SNP-injected mice .
	manualset3
174467	4	410721	13	NULL	NULL	0	NULL	catalase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of lipid peroxidation and the activity of catalase , glutathione peroxidase ( GPx ) , glutathione S-transferase ( GST ) and glutathione reductase ( GR ) were carried out in brain homogenates of SNP-injected mice .
	manualset3
174468	5	410721	13	NULL	NULL	0	NULL	glutathione peroxidase ( GPx )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of lipid peroxidation and the activity of catalase , glutathione peroxidase ( GPx ) , glutathione S-transferase ( GST ) and glutathione reductase ( GR ) were carried out in brain homogenates of SNP-injected mice .
	manualset3
174469	6	410721	13	NULL	NULL	0	NULL	 glutathione S-transferase ( GST ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of lipid peroxidation and the activity of catalase , glutathione peroxidase ( GPx ) , glutathione S-transferase ( GST ) and glutathione reductase ( GR ) were carried out in brain homogenates of SNP-injected mice .
	manualset3
174470	7	410721	13	NULL	NULL	0	NULL	 glutathione reductase ( GR ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of lipid peroxidation and the activity of catalase , glutathione peroxidase ( GPx ) , glutathione S-transferase ( GST ) and glutathione reductase ( GR ) were carried out in brain homogenates of SNP-injected mice .
	manualset3
174471	8	410721	13	NULL	NULL	NULL	NULL	brain homogenates 	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The levels of lipid peroxidation and the activity of catalase , glutathione peroxidase ( GPx ) , glutathione S-transferase ( GST ) and glutathione reductase ( GR ) were carried out in brain homogenates of SNP-injected mice .
	manualset3
174472	9	410721	13	NULL	NULL	0	NULL	 SNP-injected mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of lipid peroxidation and the activity of catalase , glutathione peroxidase ( GPx ) , glutathione S-transferase ( GST ) and glutathione reductase ( GR ) were carried out in brain homogenates of SNP-injected mice .
	manualset3
174473	1	410722	13	NULL	NULL	0	NULL	levels 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of nirB and ntcB transcripts were low in cells growing on ammonium and increased upon transfer of ammonium-grown cells to nitrate-containing medium .
	manualset3
174474	2	410722	13	NULL	NULL	0	NULL	nirB transcripts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of nirB and ntcB transcripts were low in cells growing on ammonium and increased upon transfer of ammonium-grown cells to nitrate-containing medium .
	manualset3
174475	3	410722	13	NULL	NULL	0	NULL	ntcB transcripts 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of nirB and ntcB transcripts were low in cells growing on ammonium and increased upon transfer of ammonium-grown cells to nitrate-containing medium .
	manualset3
174476	4	410722	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of nirB and ntcB transcripts were low in cells growing on ammonium and increased upon transfer of ammonium-grown cells to nitrate-containing medium .
	manualset3
174477	5	410722	13	NULL	NULL	0	NULL	ammonium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of nirB and ntcB transcripts were low in cells growing on ammonium and increased upon transfer of ammonium-grown cells to nitrate-containing medium .
	manualset3
174478	6	410722	13	NULL	NULL	0	NULL	transfer	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of nirB and ntcB transcripts were low in cells growing on ammonium and increased upon transfer of ammonium-grown cells to nitrate-containing medium .
	manualset3
174479	7	410722	13	NULL	NULL	0	NULL	ammonium-grown cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of nirB and ntcB transcripts were low in cells growing on ammonium and increased upon transfer of ammonium-grown cells to nitrate-containing medium .
	manualset3
174480	8	410722	13	NULL	NULL	0	NULL	nitrate-containing medium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of nirB and ntcB transcripts were low in cells growing on ammonium and increased upon transfer of ammonium-grown cells to nitrate-containing medium .
	manualset3
174481	1	410723	13	NULL	NULL	0	NULL	levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of the analyzed chlorinated pesticides in the fjord surface waters were found to be low compared to earlier studies .
	manualset3
174482	2	410723	13	NULL	NULL	0	NULL	 chlorinated pesticides 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of the analyzed chlorinated pesticides in the fjord surface waters were found to be low compared to earlier studies .
	manualset3
174483	3	410723	13	NULL	NULL	0	NULL	fjord surface waters 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of the analyzed chlorinated pesticides in the fjord surface waters were found to be low compared to earlier studies .
	manualset3
174484	4	410723	13	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The levels of the analyzed chlorinated pesticides in the fjord surface waters were found to be low compared to earlier studies .
	manualset3
174485	1	410724	13	NULL	NULL	0	NULL	oligosaccharide phosphates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The liberated oligosaccharide phosphates were studied by NMR spectroscopy and by electrospray and fast atom bombardment mass spectrometry .
	manualset3
174486	2	410724	13	NULL	NULL	0	NULL	 NMR spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The liberated oligosaccharide phosphates were studied by NMR spectroscopy and by electrospray and fast atom bombardment mass spectrometry .
	manualset3
174487	3	410724	13	NULL	NULL	0	NULL	electrospray	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The liberated oligosaccharide phosphates were studied by NMR spectroscopy and by electrospray and fast atom bombardment mass spectrometry .
	manualset3
174488	4	410724	13	NULL	NULL	0	NULL	fast atom bombardment mass spectrometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The liberated oligosaccharide phosphates were studied by NMR spectroscopy and by electrospray and fast atom bombardment mass spectrometry .
	manualset3
174489	1	410725	13	NULL	NULL	0	NULL	 library	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The library was screened with an oligonucleotide probe constructed from the putative zinc-binding region of fibroblast collagenase .
	manualset3
174490	2	410725	13	NULL	NULL	0	NULL	oligonucleotide probe	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The library was screened with an oligonucleotide probe constructed from the putative zinc-binding region of fibroblast collagenase .
	manualset3
174491	3	410725	13	NULL	NULL	0	NULL	putative zinc-binding region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The library was screened with an oligonucleotide probe constructed from the putative zinc-binding region of fibroblast collagenase .
	manualset3
174492	4	410725	13	NULL	NULL	0	NULL	fibroblast collagenase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The library was screened with an oligonucleotide probe constructed from the putative zinc-binding region of fibroblast collagenase .
	manualset3
174493	1	410726	13	NULL	NULL	0	NULL	 lice specimens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The lice specimens were cleared in 10 % of KOH until they were transparent .
	manualset3
174494	2	410726	13	NULL	NULL	0	NULL	10 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The lice specimens were cleared in 10 % of KOH until they were transparent .
	manualset3
174495	3	410726	13	NULL	NULL	0	NULL	KOH	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The lice specimens were cleared in 10 % of KOH until they were transparent .
	manualset3
174496	1	410727	13	NULL	NULL	0	NULL	 licensure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The licensure of hygienists : a few surprises .
	manualset3
174497	2	410727	13	NULL	NULL	0	NULL	hygienists 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The licensure of hygienists : a few surprises .
	manualset3
174498	3	410727	13	NULL	NULL	0	NULL	surprises	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The licensure of hygienists : a few surprises .
	manualset3
174499	1	410728	13	NULL	NULL	0	NULL	ligK gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The ligK gene consists of a 684-bp open reading frame encoding a polypeptide with a molecular mass of 24 , 131 Da .
	manualset3
174500	2	410728	13	NULL	NULL	0	NULL	684-bp open reading frame	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The ligK gene consists of a 684-bp open reading frame encoding a polypeptide with a molecular mass of 24 , 131 Da .
	manualset3
174501	3	410728	13	NULL	NULL	0	NULL	polypeptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The ligK gene consists of a 684-bp open reading frame encoding a polypeptide with a molecular mass of 24 , 131 Da .
	manualset3
174502	4	410728	13	NULL	NULL	0	NULL	molecular mass of 24 , 131 Da	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ligK gene consists of a 684-bp open reading frame encoding a polypeptide with a molecular mass of 24 , 131 Da .
	manualset3
174503	1	410729	13	NULL	NULL	0	NULL	light fraction	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The light fraction was essentially composed of mitochondria banded at a density of about 1.06 g/ml .
	manualset3
174504	2	410729	13	NULL	NULL	0	NULL	mitochondria 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The light fraction was essentially composed of mitochondria banded at a density of about 1.06 g/ml .
	manualset3
174505	3	410729	13	NULL	NULL	0	NULL	density	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The light fraction was essentially composed of mitochondria banded at a density of about 1.06 g/ml .
	manualset3
174506	4	410729	13	NULL	NULL	0	NULL	1.06 g/ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The light fraction was essentially composed of mitochondria banded at a density of about 1.06 g/ml .
	manualset3
174507	1	410730	13	NULL	NULL	0	NULL	likelihood 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The likelihood of complications was closely related to the radiation dosage .
	manualset3
174508	2	410730	13	NULL	NULL	0	NULL	complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The likelihood of complications was closely related to the radiation dosage .
	manualset3
174509	3	410730	13	NULL	NULL	0	NULL	radiation dosage	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The likelihood of complications was closely related to the radiation dosage .
	manualset3
174510	1	410731	13	NULL	NULL	0	NULL	total	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 507 Italian heavy pigs , supplied by two farms , were loaded by ramp or lift and transported unmixed for 35-55 min to the abattoir at a stocking density of either & lt ; 0.4 or & gt ; 0.6 m ( 2 ) per 100 kg pigs .
	manualset3
174511	2	410731	13	NULL	NULL	0	NULL	507 Italian heavy pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 507 Italian heavy pigs , supplied by two farms , were loaded by ramp or lift and transported unmixed for 35-55 min to the abattoir at a stocking density of either & lt ; 0.4 or & gt ; 0.6 m ( 2 ) per 100 kg pigs .
	manualset3
174512	3	410731	13	NULL	NULL	0	NULL	two farms	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 507 Italian heavy pigs , supplied by two farms , were loaded by ramp or lift and transported unmixed for 35-55 min to the abattoir at a stocking density of either & lt ; 0.4 or & gt ; 0.6 m ( 2 ) per 100 kg pigs .
	manualset3
174513	4	410731	13	NULL	NULL	0	NULL	ramp	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 507 Italian heavy pigs , supplied by two farms , were loaded by ramp or lift and transported unmixed for 35-55 min to the abattoir at a stocking density of either & lt ; 0.4 or & gt ; 0.6 m ( 2 ) per 100 kg pigs .
	manualset3
174514	5	410731	13	NULL	NULL	0	NULL	lift	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 507 Italian heavy pigs , supplied by two farms , were loaded by ramp or lift and transported unmixed for 35-55 min to the abattoir at a stocking density of either & lt ; 0.4 or & gt ; 0.6 m ( 2 ) per 100 kg pigs .
	manualset3
174515	6	410731	13	NULL	NULL	0	NULL	 35-55 min 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 507 Italian heavy pigs , supplied by two farms , were loaded by ramp or lift and transported unmixed for 35-55 min to the abattoir at a stocking density of either & lt ; 0.4 or & gt ; 0.6 m ( 2 ) per 100 kg pigs .
	manualset3
174516	7	410731	13	NULL	NULL	0	NULL	abattoir	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 507 Italian heavy pigs , supplied by two farms , were loaded by ramp or lift and transported unmixed for 35-55 min to the abattoir at a stocking density of either & lt ; 0.4 or & gt ; 0.6 m ( 2 ) per 100 kg pigs .
	manualset3
174517	8	410731	13	NULL	NULL	0	NULL	 stocking density 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 507 Italian heavy pigs , supplied by two farms , were loaded by ramp or lift and transported unmixed for 35-55 min to the abattoir at a stocking density of either & lt ; 0.4 or & gt ; 0.6 m ( 2 ) per 100 kg pigs .
	manualset3
174518	9	410731	13	NULL	NULL	0	NULL	 0.4 or & gt ; 0.6 m ( 2 ) per 100 kg pigs 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 507 Italian heavy pigs , supplied by two farms , were loaded by ramp or lift and transported unmixed for 35-55 min to the abattoir at a stocking density of either & lt ; 0.4 or & gt ; 0.6 m ( 2 ) per 100 kg pigs .
	manualset3
174519	1	410732	13	NULL	NULL	0	NULL	limb length discrepancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The limb length discrepancy is oftentimes associated with functional abnormalities , such as overpronation of one foot in contradistinction to the other or imbalances within the pelvis itself .
	manualset3
174520	2	410732	13	NULL	NULL	0	NULL	functional abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The limb length discrepancy is oftentimes associated with functional abnormalities , such as overpronation of one foot in contradistinction to the other or imbalances within the pelvis itself .
	manualset3
174521	3	410732	13	NULL	NULL	0	NULL	 overpronation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The limb length discrepancy is oftentimes associated with functional abnormalities , such as overpronation of one foot in contradistinction to the other or imbalances within the pelvis itself .
	manualset3
174522	4	410732	13	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The limb length discrepancy is oftentimes associated with functional abnormalities , such as overpronation of one foot in contradistinction to the other or imbalances within the pelvis itself .
	manualset3
174523	5	410732	13	NULL	NULL	0	NULL	 foot 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The limb length discrepancy is oftentimes associated with functional abnormalities , such as overpronation of one foot in contradistinction to the other or imbalances within the pelvis itself .
	manualset3
174524	6	410732	13	NULL	NULL	0	NULL	contradistinction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The limb length discrepancy is oftentimes associated with functional abnormalities , such as overpronation of one foot in contradistinction to the other or imbalances within the pelvis itself .
	manualset3
174525	7	410732	13	NULL	NULL	0	NULL	imbalances	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The limb length discrepancy is oftentimes associated with functional abnormalities , such as overpronation of one foot in contradistinction to the other or imbalances within the pelvis itself .
	manualset3
174526	8	410732	13	NULL	NULL	0	NULL	pelvis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The limb length discrepancy is oftentimes associated with functional abnormalities , such as overpronation of one foot in contradistinction to the other or imbalances within the pelvis itself .
	manualset3
174527	1	410733	13	NULL	NULL	NULL	NULL	limit	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The limit of detection for cyclopentadiene in carbon tetrachloride solutions is 0.11 microg/ml .
	manualset3
174528	2	410733	13	NULL	NULL	0	NULL	detection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The limit of detection for cyclopentadiene in carbon tetrachloride solutions is 0.11 microg/ml .
	manualset3
174529	3	410733	13	NULL	NULL	0	NULL	cyclopentadiene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The limit of detection for cyclopentadiene in carbon tetrachloride solutions is 0.11 microg/ml .
	manualset3
174530	4	410733	13	NULL	NULL	0	NULL	carbon tetrachloride solutions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The limit of detection for cyclopentadiene in carbon tetrachloride solutions is 0.11 microg/ml .
	manualset3
174531	5	410733	13	NULL	NULL	0	NULL	0.11 microg/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The limit of detection for cyclopentadiene in carbon tetrachloride solutions is 0.11 microg/ml .
	manualset3
174532	1	410734	13	NULL	NULL	0	NULL	 limit	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The limit of detection is 7 x 10 ( -9 ) M. The selectivity obtained for homovanillic acid over other structurally related compounds buttresses the validity of this strategy of design .
	manualset3
174533	2	410734	13	NULL	NULL	0	NULL	detection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The limit of detection is 7 x 10 ( -9 ) M. The selectivity obtained for homovanillic acid over other structurally related compounds buttresses the validity of this strategy of design .
	manualset3
174534	3	410734	13	NULL	NULL	0	NULL	7 x 10 ( -9 ) M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The limit of detection is 7 x 10 ( -9 ) M. The selectivity obtained for homovanillic acid over other structurally related compounds buttresses the validity of this strategy of design .
	manualset3
174535	4	410734	13	NULL	NULL	0	NULL	selectivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The limit of detection is 7 x 10 ( -9 ) M. The selectivity obtained for homovanillic acid over other structurally related compounds buttresses the validity of this strategy of design .
	manualset3
174536	5	410734	13	NULL	NULL	0	NULL	homovanillic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The limit of detection is 7 x 10 ( -9 ) M. The selectivity obtained for homovanillic acid over other structurally related compounds buttresses the validity of this strategy of design .
	manualset3
174537	6	410734	13	NULL	NULL	0	NULL	compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The limit of detection is 7 x 10 ( -9 ) M. The selectivity obtained for homovanillic acid over other structurally related compounds buttresses the validity of this strategy of design .
	manualset3
174539	8	410734	13	NULL	NULL	0	NULL	validity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The limit of detection is 7 x 10 ( -9 ) M. The selectivity obtained for homovanillic acid over other structurally related compounds buttresses the validity of this strategy of design .
	manualset3
174540	9	410734	13	NULL	NULL	0	NULL	strategy 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The limit of detection is 7 x 10 ( -9 ) M. The selectivity obtained for homovanillic acid over other structurally related compounds buttresses the validity of this strategy of design .
	manualset3
174541	10	410734	13	NULL	NULL	0	NULL	design	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The limit of detection is 7 x 10 ( -9 ) M. The selectivity obtained for homovanillic acid over other structurally related compounds buttresses the validity of this strategy of design .
	manualset3
174542	1	410735	13	NULL	NULL	0	NULL	number	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The limited number of patients in this series called for caution in generalisation .
	manualset3
174543	2	410735	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The limited number of patients in this series called for caution in generalisation .
	manualset3
174544	3	410735	13	NULL	NULL	0	NULL	series	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The limited number of patients in this series called for caution in generalisation .
	manualset3
174545	4	410735	13	NULL	NULL	0	NULL	 caution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The limited number of patients in this series called for caution in generalisation .
	manualset3
174546	5	410735	13	NULL	NULL	0	NULL	generalisation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The limited number of patients in this series called for caution in generalisation .
	manualset3
174547	1	410736	13	NULL	NULL	0	NULL	limits 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The limits applied to those specifications need to reflect the true batch to batch consistency of the product , its nature and toxicity as well as its intended use .
	manualset3
174548	2	410736	13	NULL	NULL	0	NULL	specifications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The limits applied to those specifications need to reflect the true batch to batch consistency of the product , its nature and toxicity as well as its intended use .
	manualset3
174549	3	410736	13	NULL	NULL	0	NULL	 batch	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The limits applied to those specifications need to reflect the true batch to batch consistency of the product , its nature and toxicity as well as its intended use .
	manualset3
174550	4	410736	13	NULL	NULL	0	NULL	batch consistency	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The limits applied to those specifications need to reflect the true batch to batch consistency of the product , its nature and toxicity as well as its intended use .
	manualset3
174551	5	410736	13	NULL	NULL	NULL	NULL	product	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The limits applied to those specifications need to reflect the true batch to batch consistency of the product , its nature and toxicity as well as its intended use .
	manualset3
174552	6	410736	13	NULL	NULL	0	NULL	nature 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The limits applied to those specifications need to reflect the true batch to batch consistency of the product , its nature and toxicity as well as its intended use .
	manualset3
174553	7	410736	13	NULL	NULL	0	NULL	 toxicity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The limits applied to those specifications need to reflect the true batch to batch consistency of the product , its nature and toxicity as well as its intended use .
	manualset3
174554	8	410736	13	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The limits applied to those specifications need to reflect the true batch to batch consistency of the product , its nature and toxicity as well as its intended use .
	manualset3
174555	1	410737	13	NULL	NULL	0	NULL	limits	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The limits of polarization transfer efficiency are explored for systems consisting of three isotropically coupled spins 1/2 in the absence of relaxation .
	manualset3
174556	2	410737	13	NULL	NULL	0	NULL	polarization transfer efficiency	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The limits of polarization transfer efficiency are explored for systems consisting of three isotropically coupled spins 1/2 in the absence of relaxation .
	manualset3
174557	3	410737	13	NULL	NULL	0	NULL	systems	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The limits of polarization transfer efficiency are explored for systems consisting of three isotropically coupled spins 1/2 in the absence of relaxation .
	manualset3
174558	4	410737	13	NULL	NULL	0	NULL	three 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The limits of polarization transfer efficiency are explored for systems consisting of three isotropically coupled spins 1/2 in the absence of relaxation .
	manualset3
174559	5	410737	13	NULL	NULL	0	NULL	isotropically coupled spins 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The limits of polarization transfer efficiency are explored for systems consisting of three isotropically coupled spins 1/2 in the absence of relaxation .
	manualset3
174560	6	410737	13	NULL	NULL	0	NULL	1/2 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The limits of polarization transfer efficiency are explored for systems consisting of three isotropically coupled spins 1/2 in the absence of relaxation .
	manualset3
174561	7	410737	13	NULL	NULL	0	NULL	absence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The limits of polarization transfer efficiency are explored for systems consisting of three isotropically coupled spins 1/2 in the absence of relaxation .
	manualset3
174562	8	410737	13	NULL	NULL	0	NULL	relaxation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The limits of polarization transfer efficiency are explored for systems consisting of three isotropically coupled spins 1/2 in the absence of relaxation .
	manualset3
174563	1	410738	13	NULL	NULL	0	NULL	line-width changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The line-width changes at the AT base pairs monitor the lifetime of the coil state at these positions prior to exchange with water while the line-width changes at the GC base pairs monitor the lifetime of the helix prior to dissociation to strands .
	manualset3
174564	2	410738	13	NULL	NULL	0	NULL	AT base pairs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The line-width changes at the AT base pairs monitor the lifetime of the coil state at these positions prior to exchange with water while the line-width changes at the GC base pairs monitor the lifetime of the helix prior to dissociation to strands .
	manualset3
174565	3	410738	13	NULL	NULL	0	NULL	monitor	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The line-width changes at the AT base pairs monitor the lifetime of the coil state at these positions prior to exchange with water while the line-width changes at the GC base pairs monitor the lifetime of the helix prior to dissociation to strands .
	manualset3
174567	4	410738	13	NULL	NULL	0	NULL	lifetime	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The line-width changes at the AT base pairs monitor the lifetime of the coil state at these positions prior to exchange with water while the line-width changes at the GC base pairs monitor the lifetime of the helix prior to dissociation to strands .
	manualset3
174568	5	410738	13	NULL	NULL	0	NULL	coil state	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The line-width changes at the AT base pairs monitor the lifetime of the coil state at these positions prior to exchange with water while the line-width changes at the GC base pairs monitor the lifetime of the helix prior to dissociation to strands .
	manualset3
174569	6	410738	13	NULL	NULL	0	NULL	positions 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The line-width changes at the AT base pairs monitor the lifetime of the coil state at these positions prior to exchange with water while the line-width changes at the GC base pairs monitor the lifetime of the helix prior to dissociation to strands .
	manualset3
174570	7	410738	13	NULL	NULL	0	NULL	water 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The line-width changes at the AT base pairs monitor the lifetime of the coil state at these positions prior to exchange with water while the line-width changes at the GC base pairs monitor the lifetime of the helix prior to dissociation to strands .
	manualset3
174571	8	410738	13	NULL	NULL	0	NULL	line-width changes	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The line-width changes at the AT base pairs monitor the lifetime of the coil state at these positions prior to exchange with water while the line-width changes at the GC base pairs monitor the lifetime of the helix prior to dissociation to strands .
	manualset3
174572	9	410738	13	NULL	NULL	0	NULL	GC base pairs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The line-width changes at the AT base pairs monitor the lifetime of the coil state at these positions prior to exchange with water while the line-width changes at the GC base pairs monitor the lifetime of the helix prior to dissociation to strands .
	manualset3
174573	10	410738	13	NULL	NULL	0	NULL	monitor	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The line-width changes at the AT base pairs monitor the lifetime of the coil state at these positions prior to exchange with water while the line-width changes at the GC base pairs monitor the lifetime of the helix prior to dissociation to strands .
	manualset3
174574	11	410738	13	NULL	NULL	0	NULL	lifetime	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The line-width changes at the AT base pairs monitor the lifetime of the coil state at these positions prior to exchange with water while the line-width changes at the GC base pairs monitor the lifetime of the helix prior to dissociation to strands .
	manualset3
174575	12	410738	13	NULL	NULL	0	NULL	helix	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The line-width changes at the AT base pairs monitor the lifetime of the coil state at these positions prior to exchange with water while the line-width changes at the GC base pairs monitor the lifetime of the helix prior to dissociation to strands .
	manualset3
174576	13	410738	13	NULL	NULL	0	NULL	dissociation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The line-width changes at the AT base pairs monitor the lifetime of the coil state at these positions prior to exchange with water while the line-width changes at the GC base pairs monitor the lifetime of the helix prior to dissociation to strands .
	manualset3
174577	14	410738	13	NULL	NULL	0	NULL	 strands	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The line-width changes at the AT base pairs monitor the lifetime of the coil state at these positions prior to exchange with water while the line-width changes at the GC base pairs monitor the lifetime of the helix prior to dissociation to strands .
	manualset3
174583	1	410739	13	NULL	NULL	0	NULL	linear calibration curves	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The linear calibration curves of epothilone D and metabolite were obtained over the concentration range of 0.2-1000 ng/ml and 5.0-1000 ng/ml , respectively .
	manualset3
174585	2	410739	13	NULL	NULL	0	NULL	epothilone D	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The linear calibration curves of epothilone D and metabolite were obtained over the concentration range of 0.2-1000 ng/ml and 5.0-1000 ng/ml , respectively .
	manualset3
174586	3	410739	13	NULL	NULL	0	NULL	metabolite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The linear calibration curves of epothilone D and metabolite were obtained over the concentration range of 0.2-1000 ng/ml and 5.0-1000 ng/ml , respectively .
	manualset3
174588	4	410739	13	NULL	NULL	0	NULL	concentration range	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The linear calibration curves of epothilone D and metabolite were obtained over the concentration range of 0.2-1000 ng/ml and 5.0-1000 ng/ml , respectively .
	manualset3
174589	5	410739	13	NULL	NULL	0	NULL	0.2-1000 ng/ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The linear calibration curves of epothilone D and metabolite were obtained over the concentration range of 0.2-1000 ng/ml and 5.0-1000 ng/ml , respectively .
	manualset3
174590	6	410739	13	NULL	NULL	0	NULL	5.0-1000 ng/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The linear calibration curves of epothilone D and metabolite were obtained over the concentration range of 0.2-1000 ng/ml and 5.0-1000 ng/ml , respectively .
	manualset3
174591	1	410740	13	NULL	NULL	0	NULL	linear dynamic range	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The linear dynamic range from 0.1 to 400 g L ( -1 ) and limit of detection ( LOD ) of 0.08 g L ( -1 ) were obtained under selected ion monitoring mode .
	manualset3
174592	2	410740	13	NULL	NULL	0	NULL	0.1 to 400 g L ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The linear dynamic range from 0.1 to 400 g L ( -1 ) and limit of detection ( LOD ) of 0.08 g L ( -1 ) were obtained under selected ion monitoring mode .
	manualset3
174593	3	410740	13	NULL	NULL	0	NULL	limit of detection ( LOD )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The linear dynamic range from 0.1 to 400 g L ( -1 ) and limit of detection ( LOD ) of 0.08 g L ( -1 ) were obtained under selected ion monitoring mode .
	manualset3
174594	4	410740	13	NULL	NULL	0	NULL	0.08 g L ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The linear dynamic range from 0.1 to 400 g L ( -1 ) and limit of detection ( LOD ) of 0.08 g L ( -1 ) were obtained under selected ion monitoring mode .
	manualset3
174595	5	410740	13	NULL	NULL	0	NULL	ion	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The linear dynamic range from 0.1 to 400 g L ( -1 ) and limit of detection ( LOD ) of 0.08 g L ( -1 ) were obtained under selected ion monitoring mode .
	manualset3
174596	6	410740	13	NULL	NULL	0	NULL	monitoring mode 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The linear dynamic range from 0.1 to 400 g L ( -1 ) and limit of detection ( LOD ) of 0.08 g L ( -1 ) were obtained under selected ion monitoring mode .
	manualset3
174597	1	410741	13	NULL	NULL	0	NULL	literature analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature analysis and our own notices showed that the frequency of symptomatic epilepsy in the elderly population increased .
	manualset3
174598	2	410741	13	NULL	NULL	0	NULL	notices	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature analysis and our own notices showed that the frequency of symptomatic epilepsy in the elderly population increased .
	manualset3
174599	3	410741	13	NULL	NULL	0	NULL	frequency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature analysis and our own notices showed that the frequency of symptomatic epilepsy in the elderly population increased .
	manualset3
174600	4	410741	13	NULL	NULL	0	NULL	symptomatic epilepsy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature analysis and our own notices showed that the frequency of symptomatic epilepsy in the elderly population increased .
	manualset3
174601	5	410741	13	NULL	NULL	0	NULL	elderly population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature analysis and our own notices showed that the frequency of symptomatic epilepsy in the elderly population increased .
	manualset3
174602	1	410742	13	NULL	NULL	0	NULL	literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature demonstrates that an allergic reaction to amide local anesthetics can occur and a thorough history , intradermal testing , and subcutaneous challenge are reasonable approaches to determine a safe agent for subsequent use .
	manualset3
174603	2	410742	13	NULL	NULL	0	NULL	allergic reaction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature demonstrates that an allergic reaction to amide local anesthetics can occur and a thorough history , intradermal testing , and subcutaneous challenge are reasonable approaches to determine a safe agent for subsequent use .
	manualset3
174604	3	410742	13	NULL	NULL	0	NULL	 amide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature demonstrates that an allergic reaction to amide local anesthetics can occur and a thorough history , intradermal testing , and subcutaneous challenge are reasonable approaches to determine a safe agent for subsequent use .
	manualset3
174606	4	410742	13	NULL	NULL	0	NULL	local anesthetics 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature demonstrates that an allergic reaction to amide local anesthetics can occur and a thorough history , intradermal testing , and subcutaneous challenge are reasonable approaches to determine a safe agent for subsequent use .
	manualset3
174607	5	410742	13	NULL	NULL	0	NULL	history 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature demonstrates that an allergic reaction to amide local anesthetics can occur and a thorough history , intradermal testing , and subcutaneous challenge are reasonable approaches to determine a safe agent for subsequent use .
	manualset3
174609	6	410742	13	NULL	NULL	0	NULL	intradermal testing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature demonstrates that an allergic reaction to amide local anesthetics can occur and a thorough history , intradermal testing , and subcutaneous challenge are reasonable approaches to determine a safe agent for subsequent use .
	manualset3
174610	7	410742	13	NULL	NULL	0	NULL	subcutaneous challenge	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature demonstrates that an allergic reaction to amide local anesthetics can occur and a thorough history , intradermal testing , and subcutaneous challenge are reasonable approaches to determine a safe agent for subsequent use .
	manualset3
174611	8	410742	13	NULL	NULL	0	NULL	reasonable approaches 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature demonstrates that an allergic reaction to amide local anesthetics can occur and a thorough history , intradermal testing , and subcutaneous challenge are reasonable approaches to determine a safe agent for subsequent use .
	manualset3
174612	9	410742	13	NULL	NULL	0	NULL	agent 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature demonstrates that an allergic reaction to amide local anesthetics can occur and a thorough history , intradermal testing , and subcutaneous challenge are reasonable approaches to determine a safe agent for subsequent use .
	manualset3
174613	10	410742	13	NULL	NULL	0	NULL	use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature demonstrates that an allergic reaction to amide local anesthetics can occur and a thorough history , intradermal testing , and subcutaneous challenge are reasonable approaches to determine a safe agent for subsequent use .
	manualset3
174614	1	410743	13	NULL	NULL	0	NULL	literature 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature has shown that nonadherence to medications is a multidimensional phenomenon ; relating factors can be grouped into the following categories : health system related , social/economic , condition-related , therapy-related and patient-related factors .
	manualset3
174615	2	410743	13	NULL	NULL	0	NULL	nonadherence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature has shown that nonadherence to medications is a multidimensional phenomenon ; relating factors can be grouped into the following categories : health system related , social/economic , condition-related , therapy-related and patient-related factors .
	manualset3
174616	3	410743	13	NULL	NULL	0	NULL	medications	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature has shown that nonadherence to medications is a multidimensional phenomenon ; relating factors can be grouped into the following categories : health system related , social/economic , condition-related , therapy-related and patient-related factors .
	manualset3
174617	4	410743	13	NULL	NULL	0	NULL	multidimensional phenomenon	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature has shown that nonadherence to medications is a multidimensional phenomenon ; relating factors can be grouped into the following categories : health system related , social/economic , condition-related , therapy-related and patient-related factors .
	manualset3
174618	5	410743	13	NULL	NULL	NULL	NULL	relating factors	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The literature has shown that nonadherence to medications is a multidimensional phenomenon ; relating factors can be grouped into the following categories : health system related , social/economic , condition-related , therapy-related and patient-related factors .
	manualset3
174619	6	410743	13	NULL	NULL	0	NULL	categories	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature has shown that nonadherence to medications is a multidimensional phenomenon ; relating factors can be grouped into the following categories : health system related , social/economic , condition-related , therapy-related and patient-related factors .
	manualset3
174620	7	410743	13	NULL	NULL	NULL	NULL	health system related factors	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The literature has shown that nonadherence to medications is a multidimensional phenomenon ; relating factors can be grouped into the following categories : health system related , social/economic , condition-related , therapy-related and patient-related factors .
	manualset3
174621	8	410743	13	NULL	NULL	0	NULL	social/economic factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature has shown that nonadherence to medications is a multidimensional phenomenon ; relating factors can be grouped into the following categories : health system related , social/economic , condition-related , therapy-related and patient-related factors .
	manualset3
174623	9	410743	13	NULL	NULL	0	NULL	condition-related factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature has shown that nonadherence to medications is a multidimensional phenomenon ; relating factors can be grouped into the following categories : health system related , social/economic , condition-related , therapy-related and patient-related factors .
	manualset3
174624	10	410743	13	NULL	NULL	0	NULL	therapy-related factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature has shown that nonadherence to medications is a multidimensional phenomenon ; relating factors can be grouped into the following categories : health system related , social/economic , condition-related , therapy-related and patient-related factors .
	manualset3
174626	11	410743	13	NULL	NULL	0	NULL	patient-related factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature has shown that nonadherence to medications is a multidimensional phenomenon ; relating factors can be grouped into the following categories : health system related , social/economic , condition-related , therapy-related and patient-related factors .
	manualset3
174629	1	410744	13	NULL	NULL	0	NULL	literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature indicates that it is often associated with parietal lobe lesions .
	manualset3
174631	2	410744	13	NULL	NULL	0	NULL	parietal lobe lesions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature indicates that it is often associated with parietal lobe lesions .
	manualset3
174632	1	410745	13	NULL	NULL	0	NULL	literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature indicates that lung metastases from colorectal primaries are especially suited .
	manualset3
174633	2	410745	13	NULL	NULL	0	NULL	lung metastases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature indicates that lung metastases from colorectal primaries are especially suited .
	manualset3
174634	3	410745	13	NULL	NULL	0	NULL	colorectal primaries	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature indicates that lung metastases from colorectal primaries are especially suited .
	manualset3
174635	1	410746	13	NULL	NULL	0	NULL	literature 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature is reviewed and four similar examples are found .
	manualset3
174636	2	410746	13	NULL	NULL	0	NULL	 examples	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature is reviewed and four similar examples are found .
	manualset3
174637	1	410747	13	NULL	NULL	0	NULL	total	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 587 men recruited by availability in gay meeting places and through peer referral participated in the intervention between 1992 and 1995 .
	manualset3
174638	2	410747	13	NULL	NULL	0	NULL	587 men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 587 men recruited by availability in gay meeting places and through peer referral participated in the intervention between 1992 and 1995 .
	manualset3
174639	3	410747	13	NULL	NULL	0	NULL	availability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 587 men recruited by availability in gay meeting places and through peer referral participated in the intervention between 1992 and 1995 .
	manualset3
174640	4	410747	13	NULL	NULL	0	NULL	gay meeting places 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 587 men recruited by availability in gay meeting places and through peer referral participated in the intervention between 1992 and 1995 .
	manualset3
174642	5	410747	13	NULL	NULL	0	NULL	 peer referral	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 587 men recruited by availability in gay meeting places and through peer referral participated in the intervention between 1992 and 1995 .
	manualset3
174643	6	410747	13	NULL	NULL	0	NULL	intervention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 587 men recruited by availability in gay meeting places and through peer referral participated in the intervention between 1992 and 1995 .
	manualset3
174644	7	410747	13	NULL	NULL	0	NULL	between 1992 and 1995	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 587 men recruited by availability in gay meeting places and through peer referral participated in the intervention between 1992 and 1995 .
	manualset3
174645	1	410748	13	NULL	NULL	0	NULL	literature 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature supports surgical excision , but the reports are all Level III or IV evidence consisting largely of retrospective case series .
	manualset3
174646	2	410748	13	NULL	NULL	0	NULL	surgical excision	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature supports surgical excision , but the reports are all Level III or IV evidence consisting largely of retrospective case series .
	manualset3
174647	3	410748	13	NULL	NULL	0	NULL	reports 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature supports surgical excision , but the reports are all Level III or IV evidence consisting largely of retrospective case series .
	manualset3
174648	4	410748	13	NULL	NULL	0	NULL	Level III evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature supports surgical excision , but the reports are all Level III or IV evidence consisting largely of retrospective case series .
	manualset3
174649	5	410748	13	NULL	NULL	0	NULL	Level IV evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature supports surgical excision , but the reports are all Level III or IV evidence consisting largely of retrospective case series .
	manualset3
174650	6	410748	13	NULL	NULL	0	NULL	retrospective case series 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The literature supports surgical excision , but the reports are all Level III or IV evidence consisting largely of retrospective case series .
	manualset3
174656	1	410749	13	NULL	NULL	0	NULL	liver cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The liver cells containing the structure of their active period present a normal nucleus , glycogen granules disseminated throughout the entire cytoplasm and granular mitochondria with several peripheral cristae .
	manualset3
174657	2	410749	13	NULL	NULL	0	NULL	structure	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The liver cells containing the structure of their active period present a normal nucleus , glycogen granules disseminated throughout the entire cytoplasm and granular mitochondria with several peripheral cristae .
	manualset3
174658	3	410749	13	NULL	NULL	0	NULL	active period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The liver cells containing the structure of their active period present a normal nucleus , glycogen granules disseminated throughout the entire cytoplasm and granular mitochondria with several peripheral cristae .
	manualset3
174659	4	410749	13	NULL	NULL	0	NULL	nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The liver cells containing the structure of their active period present a normal nucleus , glycogen granules disseminated throughout the entire cytoplasm and granular mitochondria with several peripheral cristae .
	manualset3
174660	5	410749	13	NULL	NULL	0	NULL	glycogen granules	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The liver cells containing the structure of their active period present a normal nucleus , glycogen granules disseminated throughout the entire cytoplasm and granular mitochondria with several peripheral cristae .
	manualset3
174661	6	410749	13	NULL	NULL	0	NULL	cytoplasm	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The liver cells containing the structure of their active period present a normal nucleus , glycogen granules disseminated throughout the entire cytoplasm and granular mitochondria with several peripheral cristae .
	manualset3
174662	7	410749	13	NULL	NULL	0	NULL	granular mitochondria 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The liver cells containing the structure of their active period present a normal nucleus , glycogen granules disseminated throughout the entire cytoplasm and granular mitochondria with several peripheral cristae .
	manualset3
174663	8	410749	13	NULL	NULL	0	NULL	several peripheral cristae	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The liver cells containing the structure of their active period present a normal nucleus , glycogen granules disseminated throughout the entire cytoplasm and granular mitochondria with several peripheral cristae .
	manualset3
174664	1	410750	13	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The liver is an exceptional organ , not only because of its unique anatomical and physiological characteristics , but also because of its unlimited regenerative capacity .
	manualset3
174665	2	410750	13	NULL	NULL	0	NULL	exceptional organ	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The liver is an exceptional organ , not only because of its unique anatomical and physiological characteristics , but also because of its unlimited regenerative capacity .
	manualset3
174666	3	410750	13	NULL	NULL	0	NULL	anatomical characteristics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The liver is an exceptional organ , not only because of its unique anatomical and physiological characteristics , but also because of its unlimited regenerative capacity .
	manualset3
174667	4	410750	13	NULL	NULL	0	NULL	physiological characteristics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The liver is an exceptional organ , not only because of its unique anatomical and physiological characteristics , but also because of its unlimited regenerative capacity .
	manualset3
174668	5	410750	13	NULL	NULL	0	NULL	regenerative capacity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The liver is an exceptional organ , not only because of its unique anatomical and physiological characteristics , but also because of its unlimited regenerative capacity .
	manualset3
174669	1	410751	13	NULL	NULL	0	NULL	liver lipid content	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The liver lipid content in control rats also was similar to that obtained by other methods ( TG , 19.0 vs 20.6 ; PL , 24.2 vs 21.8 , CH , 2.1 vs 2.1 and CE , 1.8 vs 2.6 mg/g ) .
	manualset3
174670	2	410751	13	NULL	NULL	0	NULL	control rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The liver lipid content in control rats also was similar to that obtained by other methods ( TG , 19.0 vs 20.6 ; PL , 24.2 vs 21.8 , CH , 2.1 vs 2.1 and CE , 1.8 vs 2.6 mg/g ) .
	manualset3
174671	3	410751	13	NULL	NULL	0	NULL	 methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The liver lipid content in control rats also was similar to that obtained by other methods ( TG , 19.0 vs 20.6 ; PL , 24.2 vs 21.8 , CH , 2.1 vs 2.1 and CE , 1.8 vs 2.6 mg/g ) .
	manualset3
174672	4	410751	13	NULL	NULL	0	NULL	TG , 19.0 vs 20.6 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The liver lipid content in control rats also was similar to that obtained by other methods ( TG , 19.0 vs 20.6 ; PL , 24.2 vs 21.8 , CH , 2.1 vs 2.1 and CE , 1.8 vs 2.6 mg/g ) .
	manualset3
174673	5	410751	13	NULL	NULL	0	NULL	PL , 24.2 vs 21.8	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The liver lipid content in control rats also was similar to that obtained by other methods ( TG , 19.0 vs 20.6 ; PL , 24.2 vs 21.8 , CH , 2.1 vs 2.1 and CE , 1.8 vs 2.6 mg/g ) .
	manualset3
174674	6	410751	13	NULL	NULL	0	NULL	CH , 2.1 vs 2.1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The liver lipid content in control rats also was similar to that obtained by other methods ( TG , 19.0 vs 20.6 ; PL , 24.2 vs 21.8 , CH , 2.1 vs 2.1 and CE , 1.8 vs 2.6 mg/g ) .
	manualset3
174675	7	410751	13	NULL	NULL	0	NULL	CE , 1.8 vs 2.6 mg/g 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The liver lipid content in control rats also was similar to that obtained by other methods ( TG , 19.0 vs 20.6 ; PL , 24.2 vs 21.8 , CH , 2.1 vs 2.1 and CE , 1.8 vs 2.6 mg/g ) .
	manualset3
174676	1	410752	13	NULL	NULL	0	NULL	 loading	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The loading imposed by the deployment of the stent on the artery is involved in the restenosis process .
	manualset3
174677	2	410752	13	NULL	NULL	0	NULL	deployment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The loading imposed by the deployment of the stent on the artery is involved in the restenosis process .
	manualset3
174678	3	410752	13	NULL	NULL	0	NULL	stent 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The loading imposed by the deployment of the stent on the artery is involved in the restenosis process .
	manualset3
174679	4	410752	13	NULL	NULL	0	NULL	artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The loading imposed by the deployment of the stent on the artery is involved in the restenosis process .
	manualset3
174680	5	410752	13	NULL	NULL	0	NULL	restenosis process	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The loading imposed by the deployment of the stent on the artery is involved in the restenosis process .
	manualset3
174681	1	410753	13	NULL	NULL	0	NULL	local appearance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The local appearance of various immunoglobulin ( Ig ) isotypes in the urinary tract during ascending pyelonephritis was studied in rats experimentally infected with Corynebacterium renale .
	manualset3
174682	2	410753	13	NULL	NULL	0	NULL	various immunoglobulin ( Ig ) isotypes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The local appearance of various immunoglobulin ( Ig ) isotypes in the urinary tract during ascending pyelonephritis was studied in rats experimentally infected with Corynebacterium renale .
	manualset3
174683	3	410753	13	NULL	NULL	0	NULL	urinary tract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The local appearance of various immunoglobulin ( Ig ) isotypes in the urinary tract during ascending pyelonephritis was studied in rats experimentally infected with Corynebacterium renale .
	manualset3
174684	4	410753	13	NULL	NULL	0	NULL	ascending pyelonephritis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The local appearance of various immunoglobulin ( Ig ) isotypes in the urinary tract during ascending pyelonephritis was studied in rats experimentally infected with Corynebacterium renale .
	manualset3
174686	5	410753	13	NULL	NULL	0	NULL	 rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The local appearance of various immunoglobulin ( Ig ) isotypes in the urinary tract during ascending pyelonephritis was studied in rats experimentally infected with Corynebacterium renale .
	manualset3
174687	6	410753	13	NULL	NULL	0	NULL	Corynebacterium renale	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The local appearance of various immunoglobulin ( Ig ) isotypes in the urinary tract during ascending pyelonephritis was studied in rats experimentally infected with Corynebacterium renale .
	manualset3
174688	1	410754	13	NULL	NULL	0	NULL	local production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The local production of cobalamin-binding proteins in SS was sufficient to achieve concentrations in saliva comparable to the control group .
	manualset3
174689	2	410754	13	NULL	NULL	0	NULL	cobalamin-binding proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The local production of cobalamin-binding proteins in SS was sufficient to achieve concentrations in saliva comparable to the control group .
	manualset3
174690	3	410754	13	NULL	NULL	0	NULL	SS 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The local production of cobalamin-binding proteins in SS was sufficient to achieve concentrations in saliva comparable to the control group .
	manualset3
174691	4	410754	13	NULL	NULL	0	NULL	concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The local production of cobalamin-binding proteins in SS was sufficient to achieve concentrations in saliva comparable to the control group .
	manualset3
174692	5	410754	13	NULL	NULL	0	NULL	saliva 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The local production of cobalamin-binding proteins in SS was sufficient to achieve concentrations in saliva comparable to the control group .
	manualset3
174693	6	410754	13	NULL	NULL	0	NULL	control group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The local production of cobalamin-binding proteins in SS was sufficient to achieve concentrations in saliva comparable to the control group .
	manualset3
174694	1	410755	13	NULL	NULL	0	NULL	localization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The localization of ICP 4 , ICP 8 , DNA polymerase and alkaline exonuclease within herpes simplex virus type 1 ( HSV ) - infected cells has been examined by immunofluorescence using specific antibodies to these proteins .
	manualset3
174695	2	410755	13	NULL	NULL	0	NULL	ICP 4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The localization of ICP 4 , ICP 8 , DNA polymerase and alkaline exonuclease within herpes simplex virus type 1 ( HSV ) - infected cells has been examined by immunofluorescence using specific antibodies to these proteins .
	manualset3
174696	3	410755	13	NULL	NULL	0	NULL	ICP 8 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The localization of ICP 4 , ICP 8 , DNA polymerase and alkaline exonuclease within herpes simplex virus type 1 ( HSV ) - infected cells has been examined by immunofluorescence using specific antibodies to these proteins .
	manualset3
174697	4	410755	13	NULL	NULL	0	NULL	DNA polymerase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The localization of ICP 4 , ICP 8 , DNA polymerase and alkaline exonuclease within herpes simplex virus type 1 ( HSV ) - infected cells has been examined by immunofluorescence using specific antibodies to these proteins .
	manualset3
174698	5	410755	13	NULL	NULL	0	NULL	alkaline exonuclease	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The localization of ICP 4 , ICP 8 , DNA polymerase and alkaline exonuclease within herpes simplex virus type 1 ( HSV ) - infected cells has been examined by immunofluorescence using specific antibodies to these proteins .
	manualset3
174699	6	410755	13	NULL	NULL	0	NULL	herpes simplex virus type 1 ( HSV ) - infected cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The localization of ICP 4 , ICP 8 , DNA polymerase and alkaline exonuclease within herpes simplex virus type 1 ( HSV ) - infected cells has been examined by immunofluorescence using specific antibodies to these proteins .
	manualset3
174700	7	410755	13	NULL	NULL	0	NULL	immunofluorescence 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The localization of ICP 4 , ICP 8 , DNA polymerase and alkaline exonuclease within herpes simplex virus type 1 ( HSV ) - infected cells has been examined by immunofluorescence using specific antibodies to these proteins .
	manualset3
174701	8	410755	13	NULL	NULL	0	NULL	antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The localization of ICP 4 , ICP 8 , DNA polymerase and alkaline exonuclease within herpes simplex virus type 1 ( HSV ) - infected cells has been examined by immunofluorescence using specific antibodies to these proteins .
	manualset3
174702	9	410755	13	NULL	NULL	0	NULL	proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The localization of ICP 4 , ICP 8 , DNA polymerase and alkaline exonuclease within herpes simplex virus type 1 ( HSV ) - infected cells has been examined by immunofluorescence using specific antibodies to these proteins .
	manualset3
174703	1	410756	13	NULL	NULL	0	NULL	 localization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The localization of USP33 is broadly confined to the secretory pathway , with all variants localizing to endoplasmic reticulum-associated structures .
	manualset3
174704	2	410756	13	NULL	NULL	0	NULL	USP33	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The localization of USP33 is broadly confined to the secretory pathway , with all variants localizing to endoplasmic reticulum-associated structures .
	manualset3
174705	3	410756	13	NULL	NULL	0	NULL	secretory pathway 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The localization of USP33 is broadly confined to the secretory pathway , with all variants localizing to endoplasmic reticulum-associated structures .
	manualset3
174706	4	410756	13	NULL	NULL	0	NULL	endoplasmic reticulum-associated structures	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The localization of USP33 is broadly confined to the secretory pathway , with all variants localizing to endoplasmic reticulum-associated structures .
	manualset3
174708	1	410757	13	NULL	NULL	0	NULL	location 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The location in the spinal cord of the pathway mediating cutaneous nociceptive C fiber input to climbing fibers projecting to the forelimb area of the C3 zone in the cerebellar anterior lobe was investigated in pentobarbitone-anaesthetized cats .
	manualset3
174709	2	410757	13	NULL	NULL	0	NULL	spinal cord	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The location in the spinal cord of the pathway mediating cutaneous nociceptive C fiber input to climbing fibers projecting to the forelimb area of the C3 zone in the cerebellar anterior lobe was investigated in pentobarbitone-anaesthetized cats .
	manualset3
174711	3	410757	13	NULL	NULL	0	NULL	 pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The location in the spinal cord of the pathway mediating cutaneous nociceptive C fiber input to climbing fibers projecting to the forelimb area of the C3 zone in the cerebellar anterior lobe was investigated in pentobarbitone-anaesthetized cats .
	manualset3
174714	4	410757	13	NULL	NULL	0	NULL	nociceptive C fiber 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The location in the spinal cord of the pathway mediating cutaneous nociceptive C fiber input to climbing fibers projecting to the forelimb area of the C3 zone in the cerebellar anterior lobe was investigated in pentobarbitone-anaesthetized cats .
	manualset3
174716	5	410757	13	NULL	NULL	0	NULL	climbing fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The location in the spinal cord of the pathway mediating cutaneous nociceptive C fiber input to climbing fibers projecting to the forelimb area of the C3 zone in the cerebellar anterior lobe was investigated in pentobarbitone-anaesthetized cats .
	manualset3
174717	6	410757	13	NULL	NULL	0	NULL	forelimb area 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The location in the spinal cord of the pathway mediating cutaneous nociceptive C fiber input to climbing fibers projecting to the forelimb area of the C3 zone in the cerebellar anterior lobe was investigated in pentobarbitone-anaesthetized cats .
	manualset3
174718	7	410757	13	NULL	NULL	0	NULL	C3 zone	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The location in the spinal cord of the pathway mediating cutaneous nociceptive C fiber input to climbing fibers projecting to the forelimb area of the C3 zone in the cerebellar anterior lobe was investigated in pentobarbitone-anaesthetized cats .
	manualset3
174719	8	410757	13	NULL	NULL	0	NULL	cerebellar anterior lobe	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The location in the spinal cord of the pathway mediating cutaneous nociceptive C fiber input to climbing fibers projecting to the forelimb area of the C3 zone in the cerebellar anterior lobe was investigated in pentobarbitone-anaesthetized cats .
	manualset3
174720	9	410757	13	NULL	NULL	0	NULL	pentobarbitone-anaesthetized cats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The location in the spinal cord of the pathway mediating cutaneous nociceptive C fiber input to climbing fibers projecting to the forelimb area of the C3 zone in the cerebellar anterior lobe was investigated in pentobarbitone-anaesthetized cats .
	manualset3
174721	1	410758	13	NULL	NULL	0	NULL	location	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of the micropipette tip after bicuculline microinjection in relation to TH and PNMT immunoreactive cells was as follows : ( 1 ) TH-immunoreactive cells of the A1 cell group were visible in the same relative location as the micropipette tip , and ( 2 ) no PNMT-positive cells were noted at the sites where bicuculline elicited hypotension .
	manualset3
174722	2	410758	13	NULL	NULL	0	NULL	micropipette tip 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of the micropipette tip after bicuculline microinjection in relation to TH and PNMT immunoreactive cells was as follows : ( 1 ) TH-immunoreactive cells of the A1 cell group were visible in the same relative location as the micropipette tip , and ( 2 ) no PNMT-positive cells were noted at the sites where bicuculline elicited hypotension .
	manualset3
174723	3	410758	13	NULL	NULL	0	NULL	bicuculline microinjection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of the micropipette tip after bicuculline microinjection in relation to TH and PNMT immunoreactive cells was as follows : ( 1 ) TH-immunoreactive cells of the A1 cell group were visible in the same relative location as the micropipette tip , and ( 2 ) no PNMT-positive cells were noted at the sites where bicuculline elicited hypotension .
	manualset3
174724	4	410758	13	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of the micropipette tip after bicuculline microinjection in relation to TH and PNMT immunoreactive cells was as follows : ( 1 ) TH-immunoreactive cells of the A1 cell group were visible in the same relative location as the micropipette tip , and ( 2 ) no PNMT-positive cells were noted at the sites where bicuculline elicited hypotension .
	manualset3
174725	5	410758	13	NULL	NULL	0	NULL	TH immunoreactive cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of the micropipette tip after bicuculline microinjection in relation to TH and PNMT immunoreactive cells was as follows : ( 1 ) TH-immunoreactive cells of the A1 cell group were visible in the same relative location as the micropipette tip , and ( 2 ) no PNMT-positive cells were noted at the sites where bicuculline elicited hypotension .
	manualset3
174727	6	410758	13	NULL	NULL	0	NULL	PNMT immunoreactive cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of the micropipette tip after bicuculline microinjection in relation to TH and PNMT immunoreactive cells was as follows : ( 1 ) TH-immunoreactive cells of the A1 cell group were visible in the same relative location as the micropipette tip , and ( 2 ) no PNMT-positive cells were noted at the sites where bicuculline elicited hypotension .
	manualset3
174741	7	410758	13	NULL	NULL	0	NULL	TH-immunoreactive cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of the micropipette tip after bicuculline microinjection in relation to TH and PNMT immunoreactive cells was as follows : ( 1 ) TH-immunoreactive cells of the A1 cell group were visible in the same relative location as the micropipette tip , and ( 2 ) no PNMT-positive cells were noted at the sites where bicuculline elicited hypotension .
	manualset3
174742	8	410758	13	NULL	NULL	0	NULL	A1 cell group	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of the micropipette tip after bicuculline microinjection in relation to TH and PNMT immunoreactive cells was as follows : ( 1 ) TH-immunoreactive cells of the A1 cell group were visible in the same relative location as the micropipette tip , and ( 2 ) no PNMT-positive cells were noted at the sites where bicuculline elicited hypotension .
	manualset3
174743	9	410758	13	NULL	NULL	0	NULL	 relative location	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of the micropipette tip after bicuculline microinjection in relation to TH and PNMT immunoreactive cells was as follows : ( 1 ) TH-immunoreactive cells of the A1 cell group were visible in the same relative location as the micropipette tip , and ( 2 ) no PNMT-positive cells were noted at the sites where bicuculline elicited hypotension .
	manualset3
174744	10	410758	13	NULL	NULL	0	NULL	micropipette tip	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of the micropipette tip after bicuculline microinjection in relation to TH and PNMT immunoreactive cells was as follows : ( 1 ) TH-immunoreactive cells of the A1 cell group were visible in the same relative location as the micropipette tip , and ( 2 ) no PNMT-positive cells were noted at the sites where bicuculline elicited hypotension .
	manualset3
174745	11	410758	13	NULL	NULL	0	NULL	PNMT-positive cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of the micropipette tip after bicuculline microinjection in relation to TH and PNMT immunoreactive cells was as follows : ( 1 ) TH-immunoreactive cells of the A1 cell group were visible in the same relative location as the micropipette tip , and ( 2 ) no PNMT-positive cells were noted at the sites where bicuculline elicited hypotension .
	manualset3
174747	12	410758	13	NULL	NULL	0	NULL	sites 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of the micropipette tip after bicuculline microinjection in relation to TH and PNMT immunoreactive cells was as follows : ( 1 ) TH-immunoreactive cells of the A1 cell group were visible in the same relative location as the micropipette tip , and ( 2 ) no PNMT-positive cells were noted at the sites where bicuculline elicited hypotension .
	manualset3
174748	13	410758	13	NULL	NULL	0	NULL	bicuculline elicited hypotension	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of the micropipette tip after bicuculline microinjection in relation to TH and PNMT immunoreactive cells was as follows : ( 1 ) TH-immunoreactive cells of the A1 cell group were visible in the same relative location as the micropipette tip , and ( 2 ) no PNMT-positive cells were noted at the sites where bicuculline elicited hypotension .
	manualset3
174750	1	410759	13	NULL	NULL	0	NULL	location	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of the other epitope was determined by immunoprecipitation of actin fragments synthesized in vitro .
	manualset3
174752	2	410759	13	NULL	NULL	0	NULL	epitope 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of the other epitope was determined by immunoprecipitation of actin fragments synthesized in vitro .
	manualset3
174753	3	410759	13	NULL	NULL	0	NULL	immunoprecipitation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of the other epitope was determined by immunoprecipitation of actin fragments synthesized in vitro .
	manualset3
174754	4	410759	13	NULL	NULL	0	NULL	actin fragments 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of the other epitope was determined by immunoprecipitation of actin fragments synthesized in vitro .
	manualset3
174851	1	410760	13	NULL	NULL	0	NULL	 location 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of this oxyanion binding site in the substrate binding cleft indicates direct coupling of P +4 phosphate-primed substrate binding and catalytic activation , explains the ability of GSK3 beta to processively hyperphosphorylate substrates with Ser/Thr pentad-repeats , and suggests a mechanism for autoinhibition in which the phosphorylated N terminus binds as a competitive pseudosubstrate with phospho-Ser 9 occupying the P +4 site .
	manualset3
174853	2	410760	13	NULL	NULL	0	NULL	oxyanion binding site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of this oxyanion binding site in the substrate binding cleft indicates direct coupling of P +4 phosphate-primed substrate binding and catalytic activation , explains the ability of GSK3 beta to processively hyperphosphorylate substrates with Ser/Thr pentad-repeats , and suggests a mechanism for autoinhibition in which the phosphorylated N terminus binds as a competitive pseudosubstrate with phospho-Ser 9 occupying the P +4 site .
	manualset3
174854	3	410760	13	NULL	NULL	0	NULL	substrate binding cleft 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of this oxyanion binding site in the substrate binding cleft indicates direct coupling of P +4 phosphate-primed substrate binding and catalytic activation , explains the ability of GSK3 beta to processively hyperphosphorylate substrates with Ser/Thr pentad-repeats , and suggests a mechanism for autoinhibition in which the phosphorylated N terminus binds as a competitive pseudosubstrate with phospho-Ser 9 occupying the P +4 site .
	manualset3
174856	4	410760	13	NULL	NULL	0	NULL	coupling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of this oxyanion binding site in the substrate binding cleft indicates direct coupling of P +4 phosphate-primed substrate binding and catalytic activation , explains the ability of GSK3 beta to processively hyperphosphorylate substrates with Ser/Thr pentad-repeats , and suggests a mechanism for autoinhibition in which the phosphorylated N terminus binds as a competitive pseudosubstrate with phospho-Ser 9 occupying the P +4 site .
	manualset3
174859	5	410760	13	NULL	NULL	0	NULL	 P +4 phosphate-primed substrate	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of this oxyanion binding site in the substrate binding cleft indicates direct coupling of P +4 phosphate-primed substrate binding and catalytic activation , explains the ability of GSK3 beta to processively hyperphosphorylate substrates with Ser/Thr pentad-repeats , and suggests a mechanism for autoinhibition in which the phosphorylated N terminus binds as a competitive pseudosubstrate with phospho-Ser 9 occupying the P +4 site .
	manualset3
174860	6	410760	13	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of this oxyanion binding site in the substrate binding cleft indicates direct coupling of P +4 phosphate-primed substrate binding and catalytic activation , explains the ability of GSK3 beta to processively hyperphosphorylate substrates with Ser/Thr pentad-repeats , and suggests a mechanism for autoinhibition in which the phosphorylated N terminus binds as a competitive pseudosubstrate with phospho-Ser 9 occupying the P +4 site .
	manualset3
174861	7	410760	13	NULL	NULL	0	NULL	catalytic activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of this oxyanion binding site in the substrate binding cleft indicates direct coupling of P +4 phosphate-primed substrate binding and catalytic activation , explains the ability of GSK3 beta to processively hyperphosphorylate substrates with Ser/Thr pentad-repeats , and suggests a mechanism for autoinhibition in which the phosphorylated N terminus binds as a competitive pseudosubstrate with phospho-Ser 9 occupying the P +4 site .
	manualset3
174862	8	410760	13	NULL	NULL	0	NULL	ability 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of this oxyanion binding site in the substrate binding cleft indicates direct coupling of P +4 phosphate-primed substrate binding and catalytic activation , explains the ability of GSK3 beta to processively hyperphosphorylate substrates with Ser/Thr pentad-repeats , and suggests a mechanism for autoinhibition in which the phosphorylated N terminus binds as a competitive pseudosubstrate with phospho-Ser 9 occupying the P +4 site .
	manualset3
174864	9	410760	13	NULL	NULL	0	NULL	GSK3 beta 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of this oxyanion binding site in the substrate binding cleft indicates direct coupling of P +4 phosphate-primed substrate binding and catalytic activation , explains the ability of GSK3 beta to processively hyperphosphorylate substrates with Ser/Thr pentad-repeats , and suggests a mechanism for autoinhibition in which the phosphorylated N terminus binds as a competitive pseudosubstrate with phospho-Ser 9 occupying the P +4 site .
	manualset3
174866	10	410760	13	NULL	NULL	0	NULL	hyperphosphorylate 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of this oxyanion binding site in the substrate binding cleft indicates direct coupling of P +4 phosphate-primed substrate binding and catalytic activation , explains the ability of GSK3 beta to processively hyperphosphorylate substrates with Ser/Thr pentad-repeats , and suggests a mechanism for autoinhibition in which the phosphorylated N terminus binds as a competitive pseudosubstrate with phospho-Ser 9 occupying the P +4 site .
	manualset3
174867	11	410760	13	NULL	NULL	0	NULL	substrates	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of this oxyanion binding site in the substrate binding cleft indicates direct coupling of P +4 phosphate-primed substrate binding and catalytic activation , explains the ability of GSK3 beta to processively hyperphosphorylate substrates with Ser/Thr pentad-repeats , and suggests a mechanism for autoinhibition in which the phosphorylated N terminus binds as a competitive pseudosubstrate with phospho-Ser 9 occupying the P +4 site .
	manualset3
174869	12	410760	13	NULL	NULL	0	NULL	Ser/Thr pentad-repeats	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of this oxyanion binding site in the substrate binding cleft indicates direct coupling of P +4 phosphate-primed substrate binding and catalytic activation , explains the ability of GSK3 beta to processively hyperphosphorylate substrates with Ser/Thr pentad-repeats , and suggests a mechanism for autoinhibition in which the phosphorylated N terminus binds as a competitive pseudosubstrate with phospho-Ser 9 occupying the P +4 site .
	manualset3
174870	13	410760	13	NULL	NULL	0	NULL	mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of this oxyanion binding site in the substrate binding cleft indicates direct coupling of P +4 phosphate-primed substrate binding and catalytic activation , explains the ability of GSK3 beta to processively hyperphosphorylate substrates with Ser/Thr pentad-repeats , and suggests a mechanism for autoinhibition in which the phosphorylated N terminus binds as a competitive pseudosubstrate with phospho-Ser 9 occupying the P +4 site .
	manualset3
174872	14	410760	13	NULL	NULL	0	NULL	autoinhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of this oxyanion binding site in the substrate binding cleft indicates direct coupling of P +4 phosphate-primed substrate binding and catalytic activation , explains the ability of GSK3 beta to processively hyperphosphorylate substrates with Ser/Thr pentad-repeats , and suggests a mechanism for autoinhibition in which the phosphorylated N terminus binds as a competitive pseudosubstrate with phospho-Ser 9 occupying the P +4 site .
	manualset3
174874	15	410760	13	NULL	NULL	0	NULL	N terminus	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of this oxyanion binding site in the substrate binding cleft indicates direct coupling of P +4 phosphate-primed substrate binding and catalytic activation , explains the ability of GSK3 beta to processively hyperphosphorylate substrates with Ser/Thr pentad-repeats , and suggests a mechanism for autoinhibition in which the phosphorylated N terminus binds as a competitive pseudosubstrate with phospho-Ser 9 occupying the P +4 site .
	manualset3
174875	16	410760	13	NULL	NULL	0	NULL	competitive pseudosubstrate	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of this oxyanion binding site in the substrate binding cleft indicates direct coupling of P +4 phosphate-primed substrate binding and catalytic activation , explains the ability of GSK3 beta to processively hyperphosphorylate substrates with Ser/Thr pentad-repeats , and suggests a mechanism for autoinhibition in which the phosphorylated N terminus binds as a competitive pseudosubstrate with phospho-Ser 9 occupying the P +4 site .
	manualset3
174876	17	410760	13	NULL	NULL	0	NULL	phospho-Ser 9 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of this oxyanion binding site in the substrate binding cleft indicates direct coupling of P +4 phosphate-primed substrate binding and catalytic activation , explains the ability of GSK3 beta to processively hyperphosphorylate substrates with Ser/Thr pentad-repeats , and suggests a mechanism for autoinhibition in which the phosphorylated N terminus binds as a competitive pseudosubstrate with phospho-Ser 9 occupying the P +4 site .
	manualset3
174878	18	410760	13	NULL	NULL	0	NULL	P +4 site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The location of this oxyanion binding site in the substrate binding cleft indicates direct coupling of P +4 phosphate-primed substrate binding and catalytic activation , explains the ability of GSK3 beta to processively hyperphosphorylate substrates with Ser/Thr pentad-repeats , and suggests a mechanism for autoinhibition in which the phosphorylated N terminus binds as a competitive pseudosubstrate with phospho-Ser 9 occupying the P +4 site .
	manualset3
174881	1	410761	13	NULL	NULL	0	NULL	loci	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The loci on the Escherichia coli genome of mutations affecting the constitutive enzymes glucose-6-phosphate dehydrogenase ( zwf ) and gluconate-6-phosphate dehydrogenase ( gnd ) , and the inducible enzyme gluconate-6-phosphate dehydrase ( edd ) , were determined by conjugation and transduction experiments , chiefly by three-factor crosses .
	manualset3
174882	2	410761	13	NULL	NULL	0	NULL	Escherichia coli genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The loci on the Escherichia coli genome of mutations affecting the constitutive enzymes glucose-6-phosphate dehydrogenase ( zwf ) and gluconate-6-phosphate dehydrogenase ( gnd ) , and the inducible enzyme gluconate-6-phosphate dehydrase ( edd ) , were determined by conjugation and transduction experiments , chiefly by three-factor crosses .
	manualset3
174883	3	410761	13	NULL	NULL	0	NULL	mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The loci on the Escherichia coli genome of mutations affecting the constitutive enzymes glucose-6-phosphate dehydrogenase ( zwf ) and gluconate-6-phosphate dehydrogenase ( gnd ) , and the inducible enzyme gluconate-6-phosphate dehydrase ( edd ) , were determined by conjugation and transduction experiments , chiefly by three-factor crosses .
	manualset3
174884	4	410761	13	NULL	NULL	0	NULL	constitutive enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The loci on the Escherichia coli genome of mutations affecting the constitutive enzymes glucose-6-phosphate dehydrogenase ( zwf ) and gluconate-6-phosphate dehydrogenase ( gnd ) , and the inducible enzyme gluconate-6-phosphate dehydrase ( edd ) , were determined by conjugation and transduction experiments , chiefly by three-factor crosses .
	manualset3
174885	5	410761	13	NULL	NULL	0	NULL	glucose-6-phosphate dehydrogenase ( zwf ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The loci on the Escherichia coli genome of mutations affecting the constitutive enzymes glucose-6-phosphate dehydrogenase ( zwf ) and gluconate-6-phosphate dehydrogenase ( gnd ) , and the inducible enzyme gluconate-6-phosphate dehydrase ( edd ) , were determined by conjugation and transduction experiments , chiefly by three-factor crosses .
	manualset3
174886	6	410761	13	NULL	NULL	0	NULL	gluconate-6-phosphate dehydrogenase ( gnd )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The loci on the Escherichia coli genome of mutations affecting the constitutive enzymes glucose-6-phosphate dehydrogenase ( zwf ) and gluconate-6-phosphate dehydrogenase ( gnd ) , and the inducible enzyme gluconate-6-phosphate dehydrase ( edd ) , were determined by conjugation and transduction experiments , chiefly by three-factor crosses .
	manualset3
174887	7	410761	13	NULL	NULL	0	NULL	 enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The loci on the Escherichia coli genome of mutations affecting the constitutive enzymes glucose-6-phosphate dehydrogenase ( zwf ) and gluconate-6-phosphate dehydrogenase ( gnd ) , and the inducible enzyme gluconate-6-phosphate dehydrase ( edd ) , were determined by conjugation and transduction experiments , chiefly by three-factor crosses .
	manualset3
174888	8	410761	13	NULL	NULL	0	NULL	gluconate-6-phosphate dehydrase ( edd ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The loci on the Escherichia coli genome of mutations affecting the constitutive enzymes glucose-6-phosphate dehydrogenase ( zwf ) and gluconate-6-phosphate dehydrogenase ( gnd ) , and the inducible enzyme gluconate-6-phosphate dehydrase ( edd ) , were determined by conjugation and transduction experiments , chiefly by three-factor crosses .
	manualset3
174889	9	410761	13	NULL	NULL	0	NULL	conjugation experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The loci on the Escherichia coli genome of mutations affecting the constitutive enzymes glucose-6-phosphate dehydrogenase ( zwf ) and gluconate-6-phosphate dehydrogenase ( gnd ) , and the inducible enzyme gluconate-6-phosphate dehydrase ( edd ) , were determined by conjugation and transduction experiments , chiefly by three-factor crosses .
	manualset3
174890	10	410761	13	NULL	NULL	0	NULL	transduction experiments 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The loci on the Escherichia coli genome of mutations affecting the constitutive enzymes glucose-6-phosphate dehydrogenase ( zwf ) and gluconate-6-phosphate dehydrogenase ( gnd ) , and the inducible enzyme gluconate-6-phosphate dehydrase ( edd ) , were determined by conjugation and transduction experiments , chiefly by three-factor crosses .
	manualset3
174891	11	410761	13	NULL	NULL	0	NULL	three-factor crosses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The loci on the Escherichia coli genome of mutations affecting the constitutive enzymes glucose-6-phosphate dehydrogenase ( zwf ) and gluconate-6-phosphate dehydrogenase ( gnd ) , and the inducible enzyme gluconate-6-phosphate dehydrase ( edd ) , were determined by conjugation and transduction experiments , chiefly by three-factor crosses .
	manualset3
174893	1	410762	13	NULL	NULL	0	NULL	locus	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The locus is conserved on rat chromosome 4q24 , but the homologous region on human chromosome 7q34-q36 solely contains ABP1 .
	manualset3
174894	2	410762	13	NULL	NULL	0	NULL	rat chromosome 4q24	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The locus is conserved on rat chromosome 4q24 , but the homologous region on human chromosome 7q34-q36 solely contains ABP1 .
	manualset3
174895	3	410762	13	NULL	NULL	0	NULL	homologous region	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The locus is conserved on rat chromosome 4q24 , but the homologous region on human chromosome 7q34-q36 solely contains ABP1 .
	manualset3
174896	4	410762	13	NULL	NULL	0	NULL	human chromosome 7q34-q36	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The locus is conserved on rat chromosome 4q24 , but the homologous region on human chromosome 7q34-q36 solely contains ABP1 .
	manualset3
174897	5	410762	13	NULL	NULL	0	NULL	ABP1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The locus is conserved on rat chromosome 4q24 , but the homologous region on human chromosome 7q34-q36 solely contains ABP1 .
	manualset3
174898	1	410763	13	NULL	NULL	0	NULL	 log K ' ( Cu-milk ) values 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The log K ' ( Cu-milk ) values were 4.9 , 5.0 , 3.0 and 5.1 for A , B , C and D types of milk , respectively .
	manualset3
174899	2	410763	13	NULL	NULL	0	NULL	4.9 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The log K ' ( Cu-milk ) values were 4.9 , 5.0 , 3.0 and 5.1 for A , B , C and D types of milk , respectively .
	manualset3
174900	3	410763	13	NULL	NULL	0	NULL	5.0	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The log K ' ( Cu-milk ) values were 4.9 , 5.0 , 3.0 and 5.1 for A , B , C and D types of milk , respectively .
	manualset3
174901	4	410763	13	NULL	NULL	0	NULL	3.0	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The log K ' ( Cu-milk ) values were 4.9 , 5.0 , 3.0 and 5.1 for A , B , C and D types of milk , respectively .
	manualset3
174902	5	410763	13	NULL	NULL	0	NULL	5.1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The log K ' ( Cu-milk ) values were 4.9 , 5.0 , 3.0 and 5.1 for A , B , C and D types of milk , respectively .
	manualset3
174903	6	410763	13	NULL	NULL	0	NULL	D type of milk	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The log K ' ( Cu-milk ) values were 4.9 , 5.0 , 3.0 and 5.1 for A , B , C and D types of milk , respectively .
	manualset3
174905	7	410763	13	NULL	NULL	0	NULL	A type of milk	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The log K ' ( Cu-milk ) values were 4.9 , 5.0 , 3.0 and 5.1 for A , B , C and D types of milk , respectively .
	manualset3
174906	8	410763	13	NULL	NULL	0	NULL	B type of milk	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The log K ' ( Cu-milk ) values were 4.9 , 5.0 , 3.0 and 5.1 for A , B , C and D types of milk , respectively .
	manualset3
174908	9	410763	13	NULL	NULL	NULL	NULL	C type of milk	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The log K ' ( Cu-milk ) values were 4.9 , 5.0 , 3.0 and 5.1 for A , B , C and D types of milk , respectively .
	manualset3
174910	1	410764	13	NULL	NULL	0	NULL	log K ( ow )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The log K ( ow ) ranged from -4.6 to 5.2 .
	manualset3
174911	2	410764	13	NULL	NULL	0	NULL	-4.6 to 5.2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The log K ( ow ) ranged from -4.6 to 5.2 .
	manualset3
174912	1	410765	13	NULL	NULL	0	NULL	logarithmic order	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The logarithmic order of death prevailed until about 99.99 to 99.999 % of the organisms were destroyed , after which there was a decline in the rate of destruction .
	manualset3
174913	2	410765	13	NULL	NULL	0	NULL	death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The logarithmic order of death prevailed until about 99.99 to 99.999 % of the organisms were destroyed , after which there was a decline in the rate of destruction .
	manualset3
174914	3	410765	13	NULL	NULL	0	NULL	99.99 to 99.999 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The logarithmic order of death prevailed until about 99.99 to 99.999 % of the organisms were destroyed , after which there was a decline in the rate of destruction .
	manualset3
174915	4	410765	13	NULL	NULL	0	NULL	organisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The logarithmic order of death prevailed until about 99.99 to 99.999 % of the organisms were destroyed , after which there was a decline in the rate of destruction .
	manualset3
174917	5	410765	13	NULL	NULL	0	NULL	decline	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The logarithmic order of death prevailed until about 99.99 to 99.999 % of the organisms were destroyed , after which there was a decline in the rate of destruction .
	manualset3
174919	6	410765	13	NULL	NULL	0	NULL	 rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The logarithmic order of death prevailed until about 99.99 to 99.999 % of the organisms were destroyed , after which there was a decline in the rate of destruction .
	manualset3
174920	7	410765	13	NULL	NULL	0	NULL	destruction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The logarithmic order of death prevailed until about 99.99 to 99.999 % of the organisms were destroyed , after which there was a decline in the rate of destruction .
	manualset3
174925	1	410766	13	NULL	NULL	0	NULL	long-term care	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The long-term care marketplace : an overview .
	manualset3
174927	2	410766	13	NULL	NULL	0	NULL	marketplace 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The long-term care marketplace : an overview .
	manualset3
174928	3	410766	13	NULL	NULL	0	NULL	overview	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The long-term care marketplace : an overview .
	manualset3
174932	1	410767	13	NULL	NULL	0	NULL	long-term effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The long-term effect of potassium supplementation ( normal diet plus 96 mmol KC1/d for 8 weeks ) was evaluated in 17 patients with essential hypertension .
	manualset3
174933	2	410767	13	NULL	NULL	0	NULL	potassium supplementation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The long-term effect of potassium supplementation ( normal diet plus 96 mmol KC1/d for 8 weeks ) was evaluated in 17 patients with essential hypertension .
	manualset3
174935	3	410767	13	NULL	NULL	0	NULL	normal diet 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The long-term effect of potassium supplementation ( normal diet plus 96 mmol KC1/d for 8 weeks ) was evaluated in 17 patients with essential hypertension .
	manualset3
174937	4	410767	13	NULL	NULL	0	NULL	96 mmol KC1/d 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The long-term effect of potassium supplementation ( normal diet plus 96 mmol KC1/d for 8 weeks ) was evaluated in 17 patients with essential hypertension .
	manualset3
174938	5	410767	13	NULL	NULL	0	NULL	8 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The long-term effect of potassium supplementation ( normal diet plus 96 mmol KC1/d for 8 weeks ) was evaluated in 17 patients with essential hypertension .
	manualset3
174939	6	410767	13	NULL	NULL	0	NULL	17 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The long-term effect of potassium supplementation ( normal diet plus 96 mmol KC1/d for 8 weeks ) was evaluated in 17 patients with essential hypertension .
	manualset3
174941	7	410767	13	NULL	NULL	0	NULL	hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The long-term effect of potassium supplementation ( normal diet plus 96 mmol KC1/d for 8 weeks ) was evaluated in 17 patients with essential hypertension .
	manualset3
174944	1	410768	13	NULL	NULL	0	NULL	 long-term effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The long-term effects of internal mammary chain irradiation and its role in the vascular supply of the pedicled transverse rectus abdominis musculocutaneous flap breast reconstruction .
	manualset3
174945	2	410768	13	NULL	NULL	0	NULL	internal mammary chain irradiation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The long-term effects of internal mammary chain irradiation and its role in the vascular supply of the pedicled transverse rectus abdominis musculocutaneous flap breast reconstruction .
	manualset3
174946	3	410768	13	NULL	NULL	0	NULL	role 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The long-term effects of internal mammary chain irradiation and its role in the vascular supply of the pedicled transverse rectus abdominis musculocutaneous flap breast reconstruction .
	manualset3
174947	4	410768	13	NULL	NULL	NULL	NULL	vascular supply	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The long-term effects of internal mammary chain irradiation and its role in the vascular supply of the pedicled transverse rectus abdominis musculocutaneous flap breast reconstruction .
	manualset3
174948	5	410768	13	NULL	NULL	0	NULL	 transverse rectus abdominis musculocutaneous flap breast reconstruction	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The long-term effects of internal mammary chain irradiation and its role in the vascular supply of the pedicled transverse rectus abdominis musculocutaneous flap breast reconstruction .
	manualset3
174951	1	410769	13	NULL	NULL	0	NULL	diameter	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The longest diameter of the soma of stained dorsal root ganglion cells following capsaicin and bradykinin perfusion were significantly different from each other and from the non-labelled population ( 17.5 + / - 0.7 and 24.5 + / - 0.2 microns for capsaicin ; 23.2 + / - 0.9 and 25.5 + / - 0.4 microns for bradykinin ; labeled and non-labelled cells , respectively ) .
	manualset3
174956	2	410769	13	NULL	NULL	0	NULL	soma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The longest diameter of the soma of stained dorsal root ganglion cells following capsaicin and bradykinin perfusion were significantly different from each other and from the non-labelled population ( 17.5 + / - 0.7 and 24.5 + / - 0.2 microns for capsaicin ; 23.2 + / - 0.9 and 25.5 + / - 0.4 microns for bradykinin ; labeled and non-labelled cells , respectively ) .
	manualset3
174957	3	410769	13	NULL	NULL	0	NULL	dorsal root ganglion cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The longest diameter of the soma of stained dorsal root ganglion cells following capsaicin and bradykinin perfusion were significantly different from each other and from the non-labelled population ( 17.5 + / - 0.7 and 24.5 + / - 0.2 microns for capsaicin ; 23.2 + / - 0.9 and 25.5 + / - 0.4 microns for bradykinin ; labeled and non-labelled cells , respectively ) .
	manualset3
174958	4	410769	13	NULL	NULL	0	NULL	capsaicin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The longest diameter of the soma of stained dorsal root ganglion cells following capsaicin and bradykinin perfusion were significantly different from each other and from the non-labelled population ( 17.5 + / - 0.7 and 24.5 + / - 0.2 microns for capsaicin ; 23.2 + / - 0.9 and 25.5 + / - 0.4 microns for bradykinin ; labeled and non-labelled cells , respectively ) .
	manualset3
174959	5	410769	13	NULL	NULL	0	NULL	bradykinin 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The longest diameter of the soma of stained dorsal root ganglion cells following capsaicin and bradykinin perfusion were significantly different from each other and from the non-labelled population ( 17.5 + / - 0.7 and 24.5 + / - 0.2 microns for capsaicin ; 23.2 + / - 0.9 and 25.5 + / - 0.4 microns for bradykinin ; labeled and non-labelled cells , respectively ) .
	manualset3
174960	6	410769	13	NULL	NULL	0	NULL	perfusion 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The longest diameter of the soma of stained dorsal root ganglion cells following capsaicin and bradykinin perfusion were significantly different from each other and from the non-labelled population ( 17.5 + / - 0.7 and 24.5 + / - 0.2 microns for capsaicin ; 23.2 + / - 0.9 and 25.5 + / - 0.4 microns for bradykinin ; labeled and non-labelled cells , respectively ) .
	manualset3
174961	7	410769	13	NULL	NULL	0	NULL	non-labelled population	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The longest diameter of the soma of stained dorsal root ganglion cells following capsaicin and bradykinin perfusion were significantly different from each other and from the non-labelled population ( 17.5 + / - 0.7 and 24.5 + / - 0.2 microns for capsaicin ; 23.2 + / - 0.9 and 25.5 + / - 0.4 microns for bradykinin ; labeled and non-labelled cells , respectively ) .
	manualset3
174962	8	410769	13	NULL	NULL	0	NULL	17.5 + / - 0.7 microns	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The longest diameter of the soma of stained dorsal root ganglion cells following capsaicin and bradykinin perfusion were significantly different from each other and from the non-labelled population ( 17.5 + / - 0.7 and 24.5 + / - 0.2 microns for capsaicin ; 23.2 + / - 0.9 and 25.5 + / - 0.4 microns for bradykinin ; labeled and non-labelled cells , respectively ) .
	manualset3
174963	9	410769	13	NULL	NULL	0	NULL	24.5 + / - 0.2 microns	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The longest diameter of the soma of stained dorsal root ganglion cells following capsaicin and bradykinin perfusion were significantly different from each other and from the non-labelled population ( 17.5 + / - 0.7 and 24.5 + / - 0.2 microns for capsaicin ; 23.2 + / - 0.9 and 25.5 + / - 0.4 microns for bradykinin ; labeled and non-labelled cells , respectively ) .
	manualset3
174964	10	410769	13	NULL	NULL	0	NULL	capsaicin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The longest diameter of the soma of stained dorsal root ganglion cells following capsaicin and bradykinin perfusion were significantly different from each other and from the non-labelled population ( 17.5 + / - 0.7 and 24.5 + / - 0.2 microns for capsaicin ; 23.2 + / - 0.9 and 25.5 + / - 0.4 microns for bradykinin ; labeled and non-labelled cells , respectively ) .
	manualset3
174965	11	410769	13	NULL	NULL	0	NULL	23.2 + / - 0.9 microns	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The longest diameter of the soma of stained dorsal root ganglion cells following capsaicin and bradykinin perfusion were significantly different from each other and from the non-labelled population ( 17.5 + / - 0.7 and 24.5 + / - 0.2 microns for capsaicin ; 23.2 + / - 0.9 and 25.5 + / - 0.4 microns for bradykinin ; labeled and non-labelled cells , respectively ) .
	manualset3
174966	12	410769	13	NULL	NULL	0	NULL	25.5 + / - 0.4 microns	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The longest diameter of the soma of stained dorsal root ganglion cells following capsaicin and bradykinin perfusion were significantly different from each other and from the non-labelled population ( 17.5 + / - 0.7 and 24.5 + / - 0.2 microns for capsaicin ; 23.2 + / - 0.9 and 25.5 + / - 0.4 microns for bradykinin ; labeled and non-labelled cells , respectively ) .
	manualset3
174967	13	410769	13	NULL	NULL	0	NULL	bradykinin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The longest diameter of the soma of stained dorsal root ganglion cells following capsaicin and bradykinin perfusion were significantly different from each other and from the non-labelled population ( 17.5 + / - 0.7 and 24.5 + / - 0.2 microns for capsaicin ; 23.2 + / - 0.9 and 25.5 + / - 0.4 microns for bradykinin ; labeled and non-labelled cells , respectively ) .
	manualset3
174968	14	410769	13	NULL	NULL	0	NULL	labeled cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The longest diameter of the soma of stained dorsal root ganglion cells following capsaicin and bradykinin perfusion were significantly different from each other and from the non-labelled population ( 17.5 + / - 0.7 and 24.5 + / - 0.2 microns for capsaicin ; 23.2 + / - 0.9 and 25.5 + / - 0.4 microns for bradykinin ; labeled and non-labelled cells , respectively ) .
	manualset3
174969	15	410769	13	NULL	NULL	0	NULL	non-labelled cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The longest diameter of the soma of stained dorsal root ganglion cells following capsaicin and bradykinin perfusion were significantly different from each other and from the non-labelled population ( 17.5 + / - 0.7 and 24.5 + / - 0.2 microns for capsaicin ; 23.2 + / - 0.9 and 25.5 + / - 0.4 microns for bradykinin ; labeled and non-labelled cells , respectively ) .
	manualset3
174970	1	410770	13	NULL	NULL	0	NULL	mean survival time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The longest mean survival time occurred in patients with negative EGFr and V status and positive hormone receptor ( ER and PR ) status .
	manualset3
174971	2	410770	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The longest mean survival time occurred in patients with negative EGFr and V status and positive hormone receptor ( ER and PR ) status .
	manualset3
174972	3	410770	13	NULL	NULL	0	NULL	negative EGFr status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The longest mean survival time occurred in patients with negative EGFr and V status and positive hormone receptor ( ER and PR ) status .
	manualset3
174973	4	410770	13	NULL	NULL	0	NULL	negative V status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The longest mean survival time occurred in patients with negative EGFr and V status and positive hormone receptor ( ER and PR ) status .
	manualset3
174974	5	410770	13	NULL	NULL	0	NULL	positive hormone receptor ( ER and PR ) status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The longest mean survival time occurred in patients with negative EGFr and V status and positive hormone receptor ( ER and PR ) status .
	manualset3
175213	1	410771	13	NULL	NULL	0	NULL	looplike structures	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The looplike structures generate scaling laws in a pseudorandom DNA walk constructed from the sequence , called a Lvy flight .
	manualset3
175214	2	410771	13	NULL	NULL	0	NULL	scaling laws	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The looplike structures generate scaling laws in a pseudorandom DNA walk constructed from the sequence , called a Lvy flight .
	manualset3
175215	3	410771	13	NULL	NULL	0	NULL	pseudorandom DNA walk	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The looplike structures generate scaling laws in a pseudorandom DNA walk constructed from the sequence , called a Lvy flight .
	manualset3
175216	4	410771	13	NULL	NULL	0	NULL	sequence 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The looplike structures generate scaling laws in a pseudorandom DNA walk constructed from the sequence , called a Lvy flight .
	manualset3
175217	5	410771	13	NULL	NULL	NULL	NULL	Lvy flight	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The looplike structures generate scaling laws in a pseudorandom DNA walk constructed from the sequence , called a Lvy flight .
	manualset3
175218	1	410772	13	NULL	NULL	0	NULL	loss 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The loss of Jhdm2a function results in obesity and hyperlipidemia in mice .
	manualset3
175219	2	410772	13	NULL	NULL	0	NULL	Jhdm2a function 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The loss of Jhdm2a function results in obesity and hyperlipidemia in mice .
	manualset3
175220	3	410772	13	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The loss of Jhdm2a function results in obesity and hyperlipidemia in mice .
	manualset3
175221	4	410772	13	NULL	NULL	0	NULL	obesity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The loss of Jhdm2a function results in obesity and hyperlipidemia in mice .
	manualset3
175222	5	410772	13	NULL	NULL	0	NULL	hyperlipidemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The loss of Jhdm2a function results in obesity and hyperlipidemia in mice .
	manualset3
175223	6	410772	13	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The loss of Jhdm2a function results in obesity and hyperlipidemia in mice .
	manualset3
175224	1	410773	13	NULL	NULL	0	NULL	loss of sight	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The loss of sight in glaucoma is due to the permanent optic nerve damage which is the result of a chronic elevated intraocular pressure .
	manualset3
175225	2	410773	13	NULL	NULL	0	NULL	glaucoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The loss of sight in glaucoma is due to the permanent optic nerve damage which is the result of a chronic elevated intraocular pressure .
	manualset3
175226	3	410773	13	NULL	NULL	0	NULL	optic nerve damage 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The loss of sight in glaucoma is due to the permanent optic nerve damage which is the result of a chronic elevated intraocular pressure .
	manualset3
175227	4	410773	13	NULL	NULL	0	NULL	result	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The loss of sight in glaucoma is due to the permanent optic nerve damage which is the result of a chronic elevated intraocular pressure .
	manualset3
175228	5	410773	13	NULL	NULL	0	NULL	chronic elevated intraocular pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The loss of sight in glaucoma is due to the permanent optic nerve damage which is the result of a chronic elevated intraocular pressure .
	manualset3
175229	1	410774	13	NULL	NULL	0	NULL	low-energy shoulder	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The low-energy shoulder of the main visible absorption band , present in the experimental spectra for n ) 1 , is proposed to arise from spin-forbidden singlet-triplet transitions of similar MMLCT character , consistent with the observed enhancement of this feature in the spectra of the corresponding Os oligomers .
	manualset3
175230	2	410774	13	NULL	NULL	0	NULL	visible absorption band	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The low-energy shoulder of the main visible absorption band , present in the experimental spectra for n ) 1 , is proposed to arise from spin-forbidden singlet-triplet transitions of similar MMLCT character , consistent with the observed enhancement of this feature in the spectra of the corresponding Os oligomers .
	manualset3
175231	3	410774	13	NULL	NULL	0	NULL	experimental spectra	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The low-energy shoulder of the main visible absorption band , present in the experimental spectra for n ) 1 , is proposed to arise from spin-forbidden singlet-triplet transitions of similar MMLCT character , consistent with the observed enhancement of this feature in the spectra of the corresponding Os oligomers .
	manualset3
175232	4	410774	13	NULL	NULL	0	NULL	singlet-triplet transitions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The low-energy shoulder of the main visible absorption band , present in the experimental spectra for n ) 1 , is proposed to arise from spin-forbidden singlet-triplet transitions of similar MMLCT character , consistent with the observed enhancement of this feature in the spectra of the corresponding Os oligomers .
	manualset3
175233	5	410774	13	NULL	NULL	0	NULL	MMLCT character	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The low-energy shoulder of the main visible absorption band , present in the experimental spectra for n ) 1 , is proposed to arise from spin-forbidden singlet-triplet transitions of similar MMLCT character , consistent with the observed enhancement of this feature in the spectra of the corresponding Os oligomers .
	manualset3
175234	6	410774	13	NULL	NULL	0	NULL	enhancement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The low-energy shoulder of the main visible absorption band , present in the experimental spectra for n ) 1 , is proposed to arise from spin-forbidden singlet-triplet transitions of similar MMLCT character , consistent with the observed enhancement of this feature in the spectra of the corresponding Os oligomers .
	manualset3
175235	7	410774	13	NULL	NULL	0	NULL	feature	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The low-energy shoulder of the main visible absorption band , present in the experimental spectra for n ) 1 , is proposed to arise from spin-forbidden singlet-triplet transitions of similar MMLCT character , consistent with the observed enhancement of this feature in the spectra of the corresponding Os oligomers .
	manualset3
175236	8	410774	13	NULL	NULL	0	NULL	spectra	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The low-energy shoulder of the main visible absorption band , present in the experimental spectra for n ) 1 , is proposed to arise from spin-forbidden singlet-triplet transitions of similar MMLCT character , consistent with the observed enhancement of this feature in the spectra of the corresponding Os oligomers .
	manualset3
175237	9	410774	13	NULL	NULL	0	NULL	Os oligomers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The low-energy shoulder of the main visible absorption band , present in the experimental spectra for n ) 1 , is proposed to arise from spin-forbidden singlet-triplet transitions of similar MMLCT character , consistent with the observed enhancement of this feature in the spectra of the corresponding Os oligomers .
	manualset3
175238	1	410775	13	NULL	NULL	0	NULL	low-stringency single specific primer-polymerase chain reaction ( LSSP-PCR )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The low-stringency single specific primer-polymerase chain reaction ( LSSP-PCR ) has been a sensitive and informative technique that uses the variable region of kinetoplast DNA minicircles as a genetic marker , allowing detection of DNA sequence variation .
	manualset3
175239	2	410775	13	NULL	NULL	0	NULL	sensitive technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The low-stringency single specific primer-polymerase chain reaction ( LSSP-PCR ) has been a sensitive and informative technique that uses the variable region of kinetoplast DNA minicircles as a genetic marker , allowing detection of DNA sequence variation .
	manualset3
175240	3	410775	13	NULL	NULL	0	NULL	informative technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The low-stringency single specific primer-polymerase chain reaction ( LSSP-PCR ) has been a sensitive and informative technique that uses the variable region of kinetoplast DNA minicircles as a genetic marker , allowing detection of DNA sequence variation .
	manualset3
175241	4	410775	13	NULL	NULL	0	NULL	variable region 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The low-stringency single specific primer-polymerase chain reaction ( LSSP-PCR ) has been a sensitive and informative technique that uses the variable region of kinetoplast DNA minicircles as a genetic marker , allowing detection of DNA sequence variation .
	manualset3
175242	5	410775	13	NULL	NULL	0	NULL	kinetoplast DNA minicircles	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The low-stringency single specific primer-polymerase chain reaction ( LSSP-PCR ) has been a sensitive and informative technique that uses the variable region of kinetoplast DNA minicircles as a genetic marker , allowing detection of DNA sequence variation .
	manualset3
175243	6	410775	13	NULL	NULL	0	NULL	genetic marker	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The low-stringency single specific primer-polymerase chain reaction ( LSSP-PCR ) has been a sensitive and informative technique that uses the variable region of kinetoplast DNA minicircles as a genetic marker , allowing detection of DNA sequence variation .
	manualset3
175244	7	410775	13	NULL	NULL	0	NULL	detection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The low-stringency single specific primer-polymerase chain reaction ( LSSP-PCR ) has been a sensitive and informative technique that uses the variable region of kinetoplast DNA minicircles as a genetic marker , allowing detection of DNA sequence variation .
	manualset3
175245	8	410775	13	NULL	NULL	0	NULL	DNA sequence variation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The low-stringency single specific primer-polymerase chain reaction ( LSSP-PCR ) has been a sensitive and informative technique that uses the variable region of kinetoplast DNA minicircles as a genetic marker , allowing detection of DNA sequence variation .
	manualset3
175246	1	410776	13	NULL	NULL	0	NULL	dose	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The low dose strongly induced hepatic CYP1A1 mRNA ( 25-fold ) , protein ( 12-fold ) , and activity ( ethoxyresorufin O-deethylase ( EROD ) ) ( 15-fold ) .
	manualset3
175247	2	410776	13	NULL	NULL	0	NULL	hepatic CYP1A1 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The low dose strongly induced hepatic CYP1A1 mRNA ( 25-fold ) , protein ( 12-fold ) , and activity ( ethoxyresorufin O-deethylase ( EROD ) ) ( 15-fold ) .
	manualset3
175248	3	410776	13	NULL	NULL	0	NULL	25-fold	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The low dose strongly induced hepatic CYP1A1 mRNA ( 25-fold ) , protein ( 12-fold ) , and activity ( ethoxyresorufin O-deethylase ( EROD ) ) ( 15-fold ) .
	manualset3
175249	4	410776	13	NULL	NULL	0	NULL	protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The low dose strongly induced hepatic CYP1A1 mRNA ( 25-fold ) , protein ( 12-fold ) , and activity ( ethoxyresorufin O-deethylase ( EROD ) ) ( 15-fold ) .
	manualset3
175250	5	410776	13	NULL	NULL	0	NULL	 12-fold 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The low dose strongly induced hepatic CYP1A1 mRNA ( 25-fold ) , protein ( 12-fold ) , and activity ( ethoxyresorufin O-deethylase ( EROD ) ) ( 15-fold ) .
	manualset3
175251	6	410776	13	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The low dose strongly induced hepatic CYP1A1 mRNA ( 25-fold ) , protein ( 12-fold ) , and activity ( ethoxyresorufin O-deethylase ( EROD ) ) ( 15-fold ) .
	manualset3
175252	7	410776	13	NULL	NULL	0	NULL	ethoxyresorufin O-deethylase ( EROD)	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The low dose strongly induced hepatic CYP1A1 mRNA ( 25-fold ) , protein ( 12-fold ) , and activity ( ethoxyresorufin O-deethylase ( EROD ) ) ( 15-fold ) .
	manualset3
175253	8	410776	13	NULL	NULL	0	NULL	15-fold	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The low dose strongly induced hepatic CYP1A1 mRNA ( 25-fold ) , protein ( 12-fold ) , and activity ( ethoxyresorufin O-deethylase ( EROD ) ) ( 15-fold ) .
	manualset3
175254	1	410777	13	NULL	NULL	0	NULL	low radiation dose 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The low radiation dose combined with a better spatial resolution , especially , the constant availability in a nuclear medicine department should give the preference to MAG3 .
	manualset3
175255	2	410777	13	NULL	NULL	0	NULL	spatial resolution	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The low radiation dose combined with a better spatial resolution , especially , the constant availability in a nuclear medicine department should give the preference to MAG3 .
	manualset3
175256	3	410777	13	NULL	NULL	0	NULL	availability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The low radiation dose combined with a better spatial resolution , especially , the constant availability in a nuclear medicine department should give the preference to MAG3 .
	manualset3
175257	4	410777	13	NULL	NULL	0	NULL	nuclear medicine department	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The low radiation dose combined with a better spatial resolution , especially , the constant availability in a nuclear medicine department should give the preference to MAG3 .
	manualset3
175258	5	410777	13	NULL	NULL	0	NULL	preference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The low radiation dose combined with a better spatial resolution , especially , the constant availability in a nuclear medicine department should give the preference to MAG3 .
	manualset3
175259	6	410777	13	NULL	NULL	0	NULL	MAG3	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The low radiation dose combined with a better spatial resolution , especially , the constant availability in a nuclear medicine department should give the preference to MAG3 .
	manualset3
175260	1	410778	13	NULL	NULL	0	NULL	low relapse rate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The low relapse rate for patients with an acute placebo pattern switched to placebo suggests specific drug effect played a smaller role in their initial improvement .
	manualset3
175261	2	410778	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The low relapse rate for patients with an acute placebo pattern switched to placebo suggests specific drug effect played a smaller role in their initial improvement .
	manualset3
175262	3	410778	13	NULL	NULL	0	NULL	acute placebo pattern	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The low relapse rate for patients with an acute placebo pattern switched to placebo suggests specific drug effect played a smaller role in their initial improvement .
	manualset3
175263	4	410778	13	NULL	NULL	0	NULL	placebo	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The low relapse rate for patients with an acute placebo pattern switched to placebo suggests specific drug effect played a smaller role in their initial improvement .
	manualset3
175264	5	410778	13	NULL	NULL	0	NULL	specific drug effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The low relapse rate for patients with an acute placebo pattern switched to placebo suggests specific drug effect played a smaller role in their initial improvement .
	manualset3
175265	6	410778	13	NULL	NULL	0	NULL	 role 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The low relapse rate for patients with an acute placebo pattern switched to placebo suggests specific drug effect played a smaller role in their initial improvement .
	manualset3
175266	7	410778	13	NULL	NULL	0	NULL	 improvement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The low relapse rate for patients with an acute placebo pattern switched to placebo suggests specific drug effect played a smaller role in their initial improvement .
	manualset3
175267	1	410779	13	NULL	NULL	0	NULL	affinity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The lower affinity of Met 145-oxidized calmodulin toward the target peptide correlates with experimentally observed lowering of calmodulin-activated Ca-ATPase activity when oxidized calmodulin from aged rat brains is used .
	manualset3
175268	2	410779	13	NULL	NULL	0	NULL	Met 145-oxidized calmodulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The lower affinity of Met 145-oxidized calmodulin toward the target peptide correlates with experimentally observed lowering of calmodulin-activated Ca-ATPase activity when oxidized calmodulin from aged rat brains is used .
	manualset3
175269	3	410779	13	NULL	NULL	0	NULL	target peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The lower affinity of Met 145-oxidized calmodulin toward the target peptide correlates with experimentally observed lowering of calmodulin-activated Ca-ATPase activity when oxidized calmodulin from aged rat brains is used .
	manualset3
175270	4	410779	13	NULL	NULL	0	NULL	calmodulin-activated Ca-ATPase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The lower affinity of Met 145-oxidized calmodulin toward the target peptide correlates with experimentally observed lowering of calmodulin-activated Ca-ATPase activity when oxidized calmodulin from aged rat brains is used .
	manualset3
175271	5	410779	13	NULL	NULL	0	NULL	oxidized calmodulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The lower affinity of Met 145-oxidized calmodulin toward the target peptide correlates with experimentally observed lowering of calmodulin-activated Ca-ATPase activity when oxidized calmodulin from aged rat brains is used .
	manualset3
175272	6	410779	13	NULL	NULL	0	NULL	aged rat brains	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The lower affinity of Met 145-oxidized calmodulin toward the target peptide correlates with experimentally observed lowering of calmodulin-activated Ca-ATPase activity when oxidized calmodulin from aged rat brains is used .
	manualset3
175273	1	410780	13	NULL	NULL	0	NULL	amount	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The lower amount of PsaK present in PSI * may explain its higher electrophoretic mobility .
	manualset3
175274	2	410780	13	NULL	NULL	0	NULL	 PsaK 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The lower amount of PsaK present in PSI * may explain its higher electrophoretic mobility .
	manualset3
175276	3	410780	13	NULL	NULL	0	NULL	PSI 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The lower amount of PsaK present in PSI * may explain its higher electrophoretic mobility .
	manualset3
175277	4	410780	13	NULL	NULL	0	NULL	electrophoretic mobility	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The lower amount of PsaK present in PSI * may explain its higher electrophoretic mobility .
	manualset3
175278	1	410781	13	NULL	NULL	0	NULL	lower hydrocarbons	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The lower hydrocarbons ( ethylene , ethane , and propylene ) were also converted to methane at about 300 degrees C. Conversion of benzene was also possible when other hydrocarbons were present at high concentrations .
	manualset3
175279	2	410781	13	NULL	NULL	0	NULL	ethylene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The lower hydrocarbons ( ethylene , ethane , and propylene ) were also converted to methane at about 300 degrees C. Conversion of benzene was also possible when other hydrocarbons were present at high concentrations .
	manualset3
175280	3	410781	13	NULL	NULL	0	NULL	ethane 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The lower hydrocarbons ( ethylene , ethane , and propylene ) were also converted to methane at about 300 degrees C. Conversion of benzene was also possible when other hydrocarbons were present at high concentrations .
	manualset3
175281	4	410781	13	NULL	NULL	0	NULL	propylene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The lower hydrocarbons ( ethylene , ethane , and propylene ) were also converted to methane at about 300 degrees C. Conversion of benzene was also possible when other hydrocarbons were present at high concentrations .
	manualset3
175282	5	410781	13	NULL	NULL	0	NULL	methane	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The lower hydrocarbons ( ethylene , ethane , and propylene ) were also converted to methane at about 300 degrees C. Conversion of benzene was also possible when other hydrocarbons were present at high concentrations .
	manualset3
175283	6	410781	13	NULL	NULL	0	NULL	300 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The lower hydrocarbons ( ethylene , ethane , and propylene ) were also converted to methane at about 300 degrees C. Conversion of benzene was also possible when other hydrocarbons were present at high concentrations .
	manualset3
175284	7	410781	13	NULL	NULL	0	NULL	Conversion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The lower hydrocarbons ( ethylene , ethane , and propylene ) were also converted to methane at about 300 degrees C. Conversion of benzene was also possible when other hydrocarbons were present at high concentrations .
	manualset3
175285	8	410781	13	NULL	NULL	0	NULL	benzene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The lower hydrocarbons ( ethylene , ethane , and propylene ) were also converted to methane at about 300 degrees C. Conversion of benzene was also possible when other hydrocarbons were present at high concentrations .
	manualset3
175286	9	410781	13	NULL	NULL	0	NULL	hydrocarbons	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The lower hydrocarbons ( ethylene , ethane , and propylene ) were also converted to methane at about 300 degrees C. Conversion of benzene was also possible when other hydrocarbons were present at high concentrations .
	manualset3
175287	10	410781	13	NULL	NULL	0	NULL	concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The lower hydrocarbons ( ethylene , ethane , and propylene ) were also converted to methane at about 300 degrees C. Conversion of benzene was also possible when other hydrocarbons were present at high concentrations .
	manualset3
175288	1	410782	13	NULL	NULL	0	NULL	 count rate values 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The lowest count rate values were obtained between six months and one year after operation .
	manualset3
175289	2	410782	13	NULL	NULL	0	NULL	 six months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The lowest count rate values were obtained between six months and one year after operation .
	manualset3
175290	3	410782	13	NULL	NULL	0	NULL	one year 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The lowest count rate values were obtained between six months and one year after operation .
	manualset3
175291	4	410782	13	NULL	NULL	0	NULL	operation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The lowest count rate values were obtained between six months and one year after operation .
	manualset3
175292	1	410783	13	NULL	NULL	0	NULL	 lowest detection rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The lowest detection rate was in the 0 % ( positive rate , 15.2 % ) and the 10 % propylene glycol ( positive rate , 12.2 % ) .
	manualset3
175293	2	410783	13	NULL	NULL	0	NULL	0 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The lowest detection rate was in the 0 % ( positive rate , 15.2 % ) and the 10 % propylene glycol ( positive rate , 12.2 % ) .
	manualset3
175294	3	410783	13	NULL	NULL	0	NULL	positive rate , 15.2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The lowest detection rate was in the 0 % ( positive rate , 15.2 % ) and the 10 % propylene glycol ( positive rate , 12.2 % ) .
	manualset3
175295	4	410783	13	NULL	NULL	0	NULL	10 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The lowest detection rate was in the 0 % ( positive rate , 15.2 % ) and the 10 % propylene glycol ( positive rate , 12.2 % ) .
	manualset3
175296	5	410783	13	NULL	NULL	0	NULL	propylene glycol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The lowest detection rate was in the 0 % ( positive rate , 15.2 % ) and the 10 % propylene glycol ( positive rate , 12.2 % ) .
	manualset3
175297	6	410783	13	NULL	NULL	0	NULL	positive rate , 12.2 %	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The lowest detection rate was in the 0 % ( positive rate , 15.2 % ) and the 10 % propylene glycol ( positive rate , 12.2 % ) .
	manualset3
175298	1	410784	13	NULL	NULL	0	NULL	lowest doses 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The lowest doses of angiotensin II ( 25 and 50 micrograms/kg SC ) had no significant effect on either water intake or urine output .
	manualset3
175299	2	410784	13	NULL	NULL	0	NULL	angiotensin II	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The lowest doses of angiotensin II ( 25 and 50 micrograms/kg SC ) had no significant effect on either water intake or urine output .
	manualset3
175300	3	410784	13	NULL	NULL	0	NULL	25 micrograms/kg SC	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The lowest doses of angiotensin II ( 25 and 50 micrograms/kg SC ) had no significant effect on either water intake or urine output .
	manualset3
175301	4	410784	13	NULL	NULL	0	NULL	50 micrograms/kg SC	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The lowest doses of angiotensin II ( 25 and 50 micrograms/kg SC ) had no significant effect on either water intake or urine output .
	manualset3
175302	5	410784	13	NULL	NULL	0	NULL	effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The lowest doses of angiotensin II ( 25 and 50 micrograms/kg SC ) had no significant effect on either water intake or urine output .
	manualset3
175303	6	410784	13	NULL	NULL	0	NULL	water intake	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The lowest doses of angiotensin II ( 25 and 50 micrograms/kg SC ) had no significant effect on either water intake or urine output .
	manualset3
175304	7	410784	13	NULL	NULL	0	NULL	 urine output	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The lowest doses of angiotensin II ( 25 and 50 micrograms/kg SC ) had no significant effect on either water intake or urine output .
	manualset3
175305	1	410785	13	NULL	NULL	0	NULL	lrrk2 p. Gly2019Ser mutation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The lrrk2 p. Gly2019Ser mutation is uncommon in a Danish cohort with various neurodegenerative disorders .
	manualset3
175306	2	410785	13	NULL	NULL	0	NULL	Danish cohort 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The lrrk2 p. Gly2019Ser mutation is uncommon in a Danish cohort with various neurodegenerative disorders .
	manualset3
175307	3	410785	13	NULL	NULL	0	NULL	 neurodegenerative disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The lrrk2 p. Gly2019Ser mutation is uncommon in a Danish cohort with various neurodegenerative disorders .
	manualset3
175308	1	410786	13	NULL	NULL	0	NULL	lubricity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The lubricity of the organic residues is subsequently studied and the influence of different adsorbents on the lubricity is investigated and discussed .
	manualset3
175309	2	410786	13	NULL	NULL	0	NULL	organic residues	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The lubricity of the organic residues is subsequently studied and the influence of different adsorbents on the lubricity is investigated and discussed .
	manualset3
175310	3	410786	13	NULL	NULL	0	NULL	influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The lubricity of the organic residues is subsequently studied and the influence of different adsorbents on the lubricity is investigated and discussed .
	manualset3
175312	4	410786	13	NULL	NULL	0	NULL	adsorbents 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The lubricity of the organic residues is subsequently studied and the influence of different adsorbents on the lubricity is investigated and discussed .
	manualset3
175313	5	410786	13	NULL	NULL	0	NULL	lubricity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The lubricity of the organic residues is subsequently studied and the influence of different adsorbents on the lubricity is investigated and discussed .
	manualset3
175314	1	410787	13	NULL	NULL	0	NULL	lumbar disc	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The lumbar disc and its imitators .
	manualset3
175315	2	410787	13	NULL	NULL	0	NULL	imitators	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The lumbar disc and its imitators .
	manualset3
175316	1	410788	13	NULL	NULL	0	NULL	 luminescence quantum yield	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The luminescence quantum yield for the Eu ( 3 + ) complex is 0.18 .
	manualset3
175317	2	410788	13	NULL	NULL	0	NULL	Eu ( 3 + ) complex	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The luminescence quantum yield for the Eu ( 3 + ) complex is 0.18 .
	manualset3
175318	3	410788	13	NULL	NULL	0	NULL	 0.18	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The luminescence quantum yield for the Eu ( 3 + ) complex is 0.18 .
	manualset3
175319	1	410789	13	NULL	NULL	0	NULL	lung ball 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The lung ball is a special type of pulmonary aspergillosis ( PA ) occurring often after chemotherapy for leukemia .
	manualset3
175320	2	410789	13	NULL	NULL	0	NULL	special type	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The lung ball is a special type of pulmonary aspergillosis ( PA ) occurring often after chemotherapy for leukemia .
	manualset3
175321	3	410789	13	NULL	NULL	0	NULL	 pulmonary aspergillosis ( PA ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The lung ball is a special type of pulmonary aspergillosis ( PA ) occurring often after chemotherapy for leukemia .
	manualset3
175322	4	410789	13	NULL	NULL	0	NULL	chemotherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The lung ball is a special type of pulmonary aspergillosis ( PA ) occurring often after chemotherapy for leukemia .
	manualset3
175323	5	410789	13	NULL	NULL	0	NULL	leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The lung ball is a special type of pulmonary aspergillosis ( PA ) occurring often after chemotherapy for leukemia .
	manualset3
175324	1	410790	13	NULL	NULL	0	NULL	lung	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The lung is constantly exposed to the environment and its microbial components .
	manualset3
175325	2	410790	13	NULL	NULL	0	NULL	environment	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The lung is constantly exposed to the environment and its microbial components .
	manualset3
175326	3	410790	13	NULL	NULL	0	NULL	microbial components	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The lung is constantly exposed to the environment and its microbial components .
	manualset3
175327	1	410791	13	NULL	NULL	0	NULL	luteolytic activity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The luteolytic activity of oxymetholone , and anabolic steroid , has been evaluated in 10 women .
	manualset3
175328	2	410791	13	NULL	NULL	0	NULL	oxymetholone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The luteolytic activity of oxymetholone , and anabolic steroid , has been evaluated in 10 women .
	manualset3
175329	3	410791	13	NULL	NULL	0	NULL	anabolic steroid	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The luteolytic activity of oxymetholone , and anabolic steroid , has been evaluated in 10 women .
	manualset3
175330	4	410791	13	NULL	NULL	0	NULL	10 women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The luteolytic activity of oxymetholone , and anabolic steroid , has been evaluated in 10 women .
	manualset3
175331	1	410792	13	NULL	NULL	0	NULL	lymphocyte transformation test	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The lymphocyte transformation test with the chlamydia antigen was positive in 72 % of cases .
	manualset3
175332	2	410792	13	NULL	NULL	0	NULL	chlamydia antigen 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The lymphocyte transformation test with the chlamydia antigen was positive in 72 % of cases .
	manualset3
175333	3	410792	13	NULL	NULL	0	NULL	72 % of cases	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The lymphocyte transformation test with the chlamydia antigen was positive in 72 % of cases .
	manualset3
175350	1	410793	13	NULL	NULL	0	NULL	lymphocytic partner	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The lymphocytic partner of this hybridoma was obtained from an IDDM patient who had undetectable levels of antibodies to insulin in his serum .
	manualset3
175351	2	410793	13	NULL	NULL	0	NULL	hybridoma	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The lymphocytic partner of this hybridoma was obtained from an IDDM patient who had undetectable levels of antibodies to insulin in his serum .
	manualset3
175352	3	410793	13	NULL	NULL	0	NULL	IDDM patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The lymphocytic partner of this hybridoma was obtained from an IDDM patient who had undetectable levels of antibodies to insulin in his serum .
	manualset3
175353	4	410793	13	NULL	NULL	0	NULL	levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The lymphocytic partner of this hybridoma was obtained from an IDDM patient who had undetectable levels of antibodies to insulin in his serum .
	manualset3
175354	5	410793	13	NULL	NULL	0	NULL	antibodies 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The lymphocytic partner of this hybridoma was obtained from an IDDM patient who had undetectable levels of antibodies to insulin in his serum .
	manualset3
175355	6	410793	13	NULL	NULL	0	NULL	insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The lymphocytic partner of this hybridoma was obtained from an IDDM patient who had undetectable levels of antibodies to insulin in his serum .
	manualset3
175357	7	410793	13	NULL	NULL	0	NULL	serum	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The lymphocytic partner of this hybridoma was obtained from an IDDM patient who had undetectable levels of antibodies to insulin in his serum .
	manualset3
175361	1	410794	13	NULL	NULL	0	NULL	lyz gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The lyz gene was cloned into an expression vector and expressed in Escherichia coli .
	manualset3
175362	2	410794	13	NULL	NULL	0	NULL	 expression vector	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The lyz gene was cloned into an expression vector and expressed in Escherichia coli .
	manualset3
175364	3	410794	13	NULL	NULL	0	NULL	Escherichia coli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The lyz gene was cloned into an expression vector and expressed in Escherichia coli .
	manualset3
175366	1	410795	13	NULL	NULL	0	NULL	m. 1555G nucleotide	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The m. 1555G nucleotide is also the wild-type allele in other mammal species and they might be at risk of suffering a mitochondrial disorder if treated with aminoglycosides .
	manualset3
175367	2	410795	13	NULL	NULL	0	NULL	wild-type allele	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The m. 1555G nucleotide is also the wild-type allele in other mammal species and they might be at risk of suffering a mitochondrial disorder if treated with aminoglycosides .
	manualset3
175368	3	410795	13	NULL	NULL	0	NULL	mammal species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The m. 1555G nucleotide is also the wild-type allele in other mammal species and they might be at risk of suffering a mitochondrial disorder if treated with aminoglycosides .
	manualset3
175369	4	410795	13	NULL	NULL	0	NULL	risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The m. 1555G nucleotide is also the wild-type allele in other mammal species and they might be at risk of suffering a mitochondrial disorder if treated with aminoglycosides .
	manualset3
175370	5	410795	13	NULL	NULL	0	NULL	mitochondrial disorder	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The m. 1555G nucleotide is also the wild-type allele in other mammal species and they might be at risk of suffering a mitochondrial disorder if treated with aminoglycosides .
	manualset3
175373	6	410795	13	NULL	NULL	0	NULL	aminoglycosides	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The m. 1555G nucleotide is also the wild-type allele in other mammal species and they might be at risk of suffering a mitochondrial disorder if treated with aminoglycosides .
	manualset3
175376	1	410796	13	NULL	NULL	0	NULL	mRNA profiles	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The mRNA and protein profiles determined by qRT-PCR and western blot in newborn , 8-week-old , and adult marmosets corroborated the immunohistochemical findings .
	manualset3
175377	2	410796	13	NULL	NULL	0	NULL	protein profiles 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The mRNA and protein profiles determined by qRT-PCR and western blot in newborn , 8-week-old , and adult marmosets corroborated the immunohistochemical findings .
	manualset3
175379	3	410796	13	NULL	NULL	0	NULL	qRT-PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The mRNA and protein profiles determined by qRT-PCR and western blot in newborn , 8-week-old , and adult marmosets corroborated the immunohistochemical findings .
	manualset3
175380	4	410796	13	NULL	NULL	0	NULL	western blot	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The mRNA and protein profiles determined by qRT-PCR and western blot in newborn , 8-week-old , and adult marmosets corroborated the immunohistochemical findings .
	manualset3
175382	5	410796	13	NULL	NULL	0	NULL	newborn marmosets	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The mRNA and protein profiles determined by qRT-PCR and western blot in newborn , 8-week-old , and adult marmosets corroborated the immunohistochemical findings .
	manualset3
175383	6	410796	13	NULL	NULL	0	NULL	8-week-old	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mRNA and protein profiles determined by qRT-PCR and western blot in newborn , 8-week-old , and adult marmosets corroborated the immunohistochemical findings .
	manualset3
175384	7	410796	13	NULL	NULL	0	NULL	adult marmosets	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The mRNA and protein profiles determined by qRT-PCR and western blot in newborn , 8-week-old , and adult marmosets corroborated the immunohistochemical findings .
	manualset3
175385	8	410796	13	NULL	NULL	0	NULL	immunohistochemical findings	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The mRNA and protein profiles determined by qRT-PCR and western blot in newborn , 8-week-old , and adult marmosets corroborated the immunohistochemical findings .
	manualset3
175386	1	410797	13	NULL	NULL	0	NULL	total 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 830 cases of animal anthrax has been recorded in 140 of 171 communities .
	manualset3
175387	2	410797	13	NULL	NULL	0	NULL	830 cases	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 830 cases of animal anthrax has been recorded in 140 of 171 communities .
	manualset3
175388	3	410797	13	NULL	NULL	0	NULL	animal anthrax	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 830 cases of animal anthrax has been recorded in 140 of 171 communities .
	manualset3
175389	4	410797	13	NULL	NULL	0	NULL	140 of 171 communities	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 830 cases of animal anthrax has been recorded in 140 of 171 communities .
	manualset3
175390	1	410798	13	NULL	NULL	0	NULL	macroscopic findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The macroscopic findings are extremely important for the diagnosis of PPE , however , this paper shows that the histopathological and/or immunohistochemical findings were also critical to identify the disease .
	manualset3
175391	2	410798	13	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The macroscopic findings are extremely important for the diagnosis of PPE , however , this paper shows that the histopathological and/or immunohistochemical findings were also critical to identify the disease .
	manualset3
175392	3	410798	13	NULL	NULL	0	NULL	PPE	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The macroscopic findings are extremely important for the diagnosis of PPE , however , this paper shows that the histopathological and/or immunohistochemical findings were also critical to identify the disease .
	manualset3
175393	4	410798	13	NULL	NULL	0	NULL	paper 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The macroscopic findings are extremely important for the diagnosis of PPE , however , this paper shows that the histopathological and/or immunohistochemical findings were also critical to identify the disease .
	manualset3
175394	5	410798	13	NULL	NULL	0	NULL	histopathological findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The macroscopic findings are extremely important for the diagnosis of PPE , however , this paper shows that the histopathological and/or immunohistochemical findings were also critical to identify the disease .
	manualset3
175395	6	410798	13	NULL	NULL	0	NULL	immunohistochemical findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The macroscopic findings are extremely important for the diagnosis of PPE , however , this paper shows that the histopathological and/or immunohistochemical findings were also critical to identify the disease .
	manualset3
175396	7	410798	13	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The macroscopic findings are extremely important for the diagnosis of PPE , however , this paper shows that the histopathological and/or immunohistochemical findings were also critical to identify the disease .
	manualset3
175397	1	410799	13	NULL	NULL	0	NULL	magnesium	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnesium content of all three types of vegetarian diets was adequate or high , ranging from 366 to 560 mg/day .
	manualset3
175398	2	410799	13	NULL	NULL	0	NULL	content	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnesium content of all three types of vegetarian diets was adequate or high , ranging from 366 to 560 mg/day .
	manualset3
175399	3	410799	13	NULL	NULL	0	NULL	three types 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnesium content of all three types of vegetarian diets was adequate or high , ranging from 366 to 560 mg/day .
	manualset3
175400	4	410799	13	NULL	NULL	0	NULL	vegetarian diets	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnesium content of all three types of vegetarian diets was adequate or high , ranging from 366 to 560 mg/day .
	manualset3
175401	5	410799	13	NULL	NULL	0	NULL	366 to 560 mg/day	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnesium content of all three types of vegetarian diets was adequate or high , ranging from 366 to 560 mg/day .
	manualset3
175402	1	410800	13	NULL	NULL	0	NULL	magnetic field sensor 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnetic field sensor ( 1.8 9 mm ) was sealed in a site 0.9 mm from the endoscope tip .
	manualset3
175403	2	410800	13	NULL	NULL	0	NULL	1.8 9 mm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnetic field sensor ( 1.8 9 mm ) was sealed in a site 0.9 mm from the endoscope tip .
	manualset3
175404	3	410800	13	NULL	NULL	0	NULL	site 0.9 mm 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnetic field sensor ( 1.8 9 mm ) was sealed in a site 0.9 mm from the endoscope tip .
	manualset3
175405	4	410800	13	NULL	NULL	0	NULL	endoscope tip	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnetic field sensor ( 1.8 9 mm ) was sealed in a site 0.9 mm from the endoscope tip .
	manualset3
175406	1	410801	13	NULL	NULL	0	NULL	magnetic parameters 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnetic parameters for the amino-protonated species R1 agree well with those extracted from previous studies of cytosine derivatives in frozen solutions and in various glasses .
	manualset3
175411	2	410801	13	NULL	NULL	0	NULL	amino-protonated species R1	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnetic parameters for the amino-protonated species R1 agree well with those extracted from previous studies of cytosine derivatives in frozen solutions and in various glasses .
	manualset3
175414	3	410801	13	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnetic parameters for the amino-protonated species R1 agree well with those extracted from previous studies of cytosine derivatives in frozen solutions and in various glasses .
	manualset3
175415	4	410801	13	NULL	NULL	0	NULL	cytosine derivatives 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnetic parameters for the amino-protonated species R1 agree well with those extracted from previous studies of cytosine derivatives in frozen solutions and in various glasses .
	manualset3
175416	5	410801	13	NULL	NULL	0	NULL	solutions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnetic parameters for the amino-protonated species R1 agree well with those extracted from previous studies of cytosine derivatives in frozen solutions and in various glasses .
	manualset3
175417	6	410801	13	NULL	NULL	0	NULL	glasses	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnetic parameters for the amino-protonated species R1 agree well with those extracted from previous studies of cytosine derivatives in frozen solutions and in various glasses .
	manualset3
175420	1	410802	13	NULL	NULL	0	NULL	magnetic spin structure factor	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnetic spin structure factor of FeF2 has been directly determined from high energy magnetic x-ray diffraction at 115 keV photon energy .
	manualset3
175422	2	410802	13	NULL	NULL	0	NULL	FeF2 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnetic spin structure factor of FeF2 has been directly determined from high energy magnetic x-ray diffraction at 115 keV photon energy .
	manualset3
175424	3	410802	13	NULL	NULL	0	NULL	high energy magnetic x-ray diffraction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnetic spin structure factor of FeF2 has been directly determined from high energy magnetic x-ray diffraction at 115 keV photon energy .
	manualset3
175425	4	410802	13	NULL	NULL	0	NULL	115 keV photon energy 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnetic spin structure factor of FeF2 has been directly determined from high energy magnetic x-ray diffraction at 115 keV photon energy .
	manualset3
175429	1	410803	13	NULL	NULL	0	NULL	 magnetic urokinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnetic urokinase dispersed in saline and exerted high fibrinolytic activity ( 13.8 X 10 ( 4 ) IU/mg protein ) , and was readily recovered from saline by magnetic force of 250 Oe .
	manualset3
175430	2	410803	13	NULL	NULL	0	NULL	saline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnetic urokinase dispersed in saline and exerted high fibrinolytic activity ( 13.8 X 10 ( 4 ) IU/mg protein ) , and was readily recovered from saline by magnetic force of 250 Oe .
	manualset3
175431	3	410803	13	NULL	NULL	0	NULL	high fibrinolytic activity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnetic urokinase dispersed in saline and exerted high fibrinolytic activity ( 13.8 X 10 ( 4 ) IU/mg protein ) , and was readily recovered from saline by magnetic force of 250 Oe .
	manualset3
175432	4	410803	13	NULL	NULL	0	NULL	13.8 X 10 ( 4 ) IU/mg protein 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnetic urokinase dispersed in saline and exerted high fibrinolytic activity ( 13.8 X 10 ( 4 ) IU/mg protein ) , and was readily recovered from saline by magnetic force of 250 Oe .
	manualset3
175433	5	410803	13	NULL	NULL	0	NULL	 saline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnetic urokinase dispersed in saline and exerted high fibrinolytic activity ( 13.8 X 10 ( 4 ) IU/mg protein ) , and was readily recovered from saline by magnetic force of 250 Oe .
	manualset3
175434	6	410803	13	NULL	NULL	0	NULL	magnetic force	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnetic urokinase dispersed in saline and exerted high fibrinolytic activity ( 13.8 X 10 ( 4 ) IU/mg protein ) , and was readily recovered from saline by magnetic force of 250 Oe .
	manualset3
175435	7	410803	13	NULL	NULL	0	NULL	250 Oe	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnetic urokinase dispersed in saline and exerted high fibrinolytic activity ( 13.8 X 10 ( 4 ) IU/mg protein ) , and was readily recovered from saline by magnetic force of 250 Oe .
	manualset3
175436	1	410804	13	NULL	NULL	0	NULL	magnitude	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of increased Rho123 accumulation in drug-treated cells was larger than that in age-matched cells .
	manualset3
175437	2	410804	13	NULL	NULL	NULL	NULL	Rho123	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The magnitude of increased Rho123 accumulation in drug-treated cells was larger than that in age-matched cells .
	manualset3
175438	3	410804	13	NULL	NULL	0	NULL	drug-treated cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of increased Rho123 accumulation in drug-treated cells was larger than that in age-matched cells .
	manualset3
175439	4	410804	13	NULL	NULL	0	NULL	age-matched cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of increased Rho123 accumulation in drug-treated cells was larger than that in age-matched cells .
	manualset3
175441	5	410804	13	NULL	NULL	0	NULL	accumulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of increased Rho123 accumulation in drug-treated cells was larger than that in age-matched cells .
	manualset3
175442	1	410805	13	NULL	NULL	0	NULL	magnitude	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of the cytotoxic response in mice with the Fb/B7 .1 / IL7/OVA cells was significantly higher than the response in mice immunized with any other cell constructs .
	manualset3
175444	2	410805	13	NULL	NULL	0	NULL	cytotoxic response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of the cytotoxic response in mice with the Fb/B7 .1 / IL7/OVA cells was significantly higher than the response in mice immunized with any other cell constructs .
	manualset3
175445	3	410805	13	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of the cytotoxic response in mice with the Fb/B7 .1 / IL7/OVA cells was significantly higher than the response in mice immunized with any other cell constructs .
	manualset3
175447	4	410805	13	NULL	NULL	0	NULL	 Fb/B7 .1 / IL7/OVA cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of the cytotoxic response in mice with the Fb/B7 .1 / IL7/OVA cells was significantly higher than the response in mice immunized with any other cell constructs .
	manualset3
175448	5	410805	13	NULL	NULL	0	NULL	response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of the cytotoxic response in mice with the Fb/B7 .1 / IL7/OVA cells was significantly higher than the response in mice immunized with any other cell constructs .
	manualset3
175449	6	410805	13	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of the cytotoxic response in mice with the Fb/B7 .1 / IL7/OVA cells was significantly higher than the response in mice immunized with any other cell constructs .
	manualset3
175450	7	410805	13	NULL	NULL	0	NULL	cell constructs 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of the cytotoxic response in mice with the Fb/B7 .1 / IL7/OVA cells was significantly higher than the response in mice immunized with any other cell constructs .
	manualset3
175451	1	410806	13	NULL	NULL	0	NULL	magnitude	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of the deviation effect ( i.e. , prolonged response time when the deviant was presented ) was relatively large in the beginning but attenuated toward the end .
	manualset3
175452	2	410806	13	NULL	NULL	0	NULL	deviation effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of the deviation effect ( i.e. , prolonged response time when the deviant was presented ) was relatively large in the beginning but attenuated toward the end .
	manualset3
175453	3	410806	13	NULL	NULL	0	NULL	response time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of the deviation effect ( i.e. , prolonged response time when the deviant was presented ) was relatively large in the beginning but attenuated toward the end .
	manualset3
175454	4	410806	13	NULL	NULL	0	NULL	beginning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of the deviation effect ( i.e. , prolonged response time when the deviant was presented ) was relatively large in the beginning but attenuated toward the end .
	manualset3
175455	5	410806	13	NULL	NULL	0	NULL	end	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of the deviation effect ( i.e. , prolonged response time when the deviant was presented ) was relatively large in the beginning but attenuated toward the end .
	manualset3
175456	1	410807	13	NULL	NULL	0	NULL	Clinical aspects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical aspects of congenital cardiopathies in adults ) .
	manualset3
175457	2	410807	13	NULL	NULL	0	NULL	congenital cardiopathies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical aspects of congenital cardiopathies in adults ) .
	manualset3
175458	3	410807	13	NULL	NULL	0	NULL	adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical aspects of congenital cardiopathies in adults ) .
	manualset3
175459	1	410808	13	NULL	NULL	0	NULL	magnitude	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of the effect was different depending on clinical subgroups : ( a ) It was greatest in patients free from angina , myocardial infarction , or new revascularization procedures at the end of follow-up ; ( b ) It was moderately reduced in patients with comorbidity ; ( c ) Patients who reported to have dyspnea or angina at rest after the latest revascularization procedure did not improve , with poor final perceived health scores .
	manualset3
175460	2	410808	13	NULL	NULL	0	NULL	effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of the effect was different depending on clinical subgroups : ( a ) It was greatest in patients free from angina , myocardial infarction , or new revascularization procedures at the end of follow-up ; ( b ) It was moderately reduced in patients with comorbidity ; ( c ) Patients who reported to have dyspnea or angina at rest after the latest revascularization procedure did not improve , with poor final perceived health scores .
	manualset3
175461	3	410808	13	NULL	NULL	0	NULL	clinical subgroups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of the effect was different depending on clinical subgroups : ( a ) It was greatest in patients free from angina , myocardial infarction , or new revascularization procedures at the end of follow-up ; ( b ) It was moderately reduced in patients with comorbidity ; ( c ) Patients who reported to have dyspnea or angina at rest after the latest revascularization procedure did not improve , with poor final perceived health scores .
	manualset3
175462	4	410808	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of the effect was different depending on clinical subgroups : ( a ) It was greatest in patients free from angina , myocardial infarction , or new revascularization procedures at the end of follow-up ; ( b ) It was moderately reduced in patients with comorbidity ; ( c ) Patients who reported to have dyspnea or angina at rest after the latest revascularization procedure did not improve , with poor final perceived health scores .
	manualset3
175463	5	410808	13	NULL	NULL	0	NULL	 angina	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of the effect was different depending on clinical subgroups : ( a ) It was greatest in patients free from angina , myocardial infarction , or new revascularization procedures at the end of follow-up ; ( b ) It was moderately reduced in patients with comorbidity ; ( c ) Patients who reported to have dyspnea or angina at rest after the latest revascularization procedure did not improve , with poor final perceived health scores .
	manualset3
175464	6	410808	13	NULL	NULL	0	NULL	myocardial infarction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of the effect was different depending on clinical subgroups : ( a ) It was greatest in patients free from angina , myocardial infarction , or new revascularization procedures at the end of follow-up ; ( b ) It was moderately reduced in patients with comorbidity ; ( c ) Patients who reported to have dyspnea or angina at rest after the latest revascularization procedure did not improve , with poor final perceived health scores .
	manualset3
175465	7	410808	13	NULL	NULL	0	NULL	revascularization procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of the effect was different depending on clinical subgroups : ( a ) It was greatest in patients free from angina , myocardial infarction , or new revascularization procedures at the end of follow-up ; ( b ) It was moderately reduced in patients with comorbidity ; ( c ) Patients who reported to have dyspnea or angina at rest after the latest revascularization procedure did not improve , with poor final perceived health scores .
	manualset3
175466	8	410808	13	NULL	NULL	0	NULL	end	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of the effect was different depending on clinical subgroups : ( a ) It was greatest in patients free from angina , myocardial infarction , or new revascularization procedures at the end of follow-up ; ( b ) It was moderately reduced in patients with comorbidity ; ( c ) Patients who reported to have dyspnea or angina at rest after the latest revascularization procedure did not improve , with poor final perceived health scores .
	manualset3
175467	9	410808	13	NULL	NULL	0	NULL	follow-up	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of the effect was different depending on clinical subgroups : ( a ) It was greatest in patients free from angina , myocardial infarction , or new revascularization procedures at the end of follow-up ; ( b ) It was moderately reduced in patients with comorbidity ; ( c ) Patients who reported to have dyspnea or angina at rest after the latest revascularization procedure did not improve , with poor final perceived health scores .
	manualset3
175468	10	410808	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of the effect was different depending on clinical subgroups : ( a ) It was greatest in patients free from angina , myocardial infarction , or new revascularization procedures at the end of follow-up ; ( b ) It was moderately reduced in patients with comorbidity ; ( c ) Patients who reported to have dyspnea or angina at rest after the latest revascularization procedure did not improve , with poor final perceived health scores .
	manualset3
175469	11	410808	13	NULL	NULL	0	NULL	comorbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of the effect was different depending on clinical subgroups : ( a ) It was greatest in patients free from angina , myocardial infarction , or new revascularization procedures at the end of follow-up ; ( b ) It was moderately reduced in patients with comorbidity ; ( c ) Patients who reported to have dyspnea or angina at rest after the latest revascularization procedure did not improve , with poor final perceived health scores .
	manualset3
175470	12	410808	13	NULL	NULL	0	NULL	Patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of the effect was different depending on clinical subgroups : ( a ) It was greatest in patients free from angina , myocardial infarction , or new revascularization procedures at the end of follow-up ; ( b ) It was moderately reduced in patients with comorbidity ; ( c ) Patients who reported to have dyspnea or angina at rest after the latest revascularization procedure did not improve , with poor final perceived health scores .
	manualset3
175471	13	410808	13	NULL	NULL	0	NULL	dyspnea	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of the effect was different depending on clinical subgroups : ( a ) It was greatest in patients free from angina , myocardial infarction , or new revascularization procedures at the end of follow-up ; ( b ) It was moderately reduced in patients with comorbidity ; ( c ) Patients who reported to have dyspnea or angina at rest after the latest revascularization procedure did not improve , with poor final perceived health scores .
	manualset3
175472	14	410808	13	NULL	NULL	0	NULL	angina	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of the effect was different depending on clinical subgroups : ( a ) It was greatest in patients free from angina , myocardial infarction , or new revascularization procedures at the end of follow-up ; ( b ) It was moderately reduced in patients with comorbidity ; ( c ) Patients who reported to have dyspnea or angina at rest after the latest revascularization procedure did not improve , with poor final perceived health scores .
	manualset3
175473	15	410808	13	NULL	NULL	0	NULL	rest	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of the effect was different depending on clinical subgroups : ( a ) It was greatest in patients free from angina , myocardial infarction , or new revascularization procedures at the end of follow-up ; ( b ) It was moderately reduced in patients with comorbidity ; ( c ) Patients who reported to have dyspnea or angina at rest after the latest revascularization procedure did not improve , with poor final perceived health scores .
	manualset3
175474	16	410808	13	NULL	NULL	0	NULL	revascularization procedure 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of the effect was different depending on clinical subgroups : ( a ) It was greatest in patients free from angina , myocardial infarction , or new revascularization procedures at the end of follow-up ; ( b ) It was moderately reduced in patients with comorbidity ; ( c ) Patients who reported to have dyspnea or angina at rest after the latest revascularization procedure did not improve , with poor final perceived health scores .
	manualset3
175475	17	410808	13	NULL	NULL	0	NULL	health scores	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The magnitude of the effect was different depending on clinical subgroups : ( a ) It was greatest in patients free from angina , myocardial infarction , or new revascularization procedures at the end of follow-up ; ( b ) It was moderately reduced in patients with comorbidity ; ( c ) Patients who reported to have dyspnea or angina at rest after the latest revascularization procedure did not improve , with poor final perceived health scores .
	manualset3
175476	1	410809	13	NULL	NULL	0	NULL	main bottlenecks 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The main bottlenecks limiting the practical applications of current magnetoresistive random access memory ( MRAM ) technology are its low storage density and high writing energy consumption .
	manualset3
175477	2	410809	13	NULL	NULL	0	NULL	practical applications 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The main bottlenecks limiting the practical applications of current magnetoresistive random access memory ( MRAM ) technology are its low storage density and high writing energy consumption .
	manualset3
175478	3	410809	13	NULL	NULL	0	NULL	magnetoresistive random access memory ( MRAM ) technology 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The main bottlenecks limiting the practical applications of current magnetoresistive random access memory ( MRAM ) technology are its low storage density and high writing energy consumption .
	manualset3
175479	4	410809	13	NULL	NULL	0	NULL	low storage density	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The main bottlenecks limiting the practical applications of current magnetoresistive random access memory ( MRAM ) technology are its low storage density and high writing energy consumption .
	manualset3
175480	5	410809	13	NULL	NULL	0	NULL	high writing energy consumption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The main bottlenecks limiting the practical applications of current magnetoresistive random access memory ( MRAM ) technology are its low storage density and high writing energy consumption .
	manualset3
175481	1	410810	13	NULL	NULL	0	NULL	main clinical features	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The main clinical features of the condition include painful and highly debilitating plantar keratoderma , hypertrophic nail dystrophy , oral leukokeratosis , and a variety of epidermal cysts .
	manualset3
175482	2	410810	13	NULL	NULL	0	NULL	condition 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The main clinical features of the condition include painful and highly debilitating plantar keratoderma , hypertrophic nail dystrophy , oral leukokeratosis , and a variety of epidermal cysts .
	manualset3
175483	3	410810	13	NULL	NULL	0	NULL	plantar keratoderma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The main clinical features of the condition include painful and highly debilitating plantar keratoderma , hypertrophic nail dystrophy , oral leukokeratosis , and a variety of epidermal cysts .
	manualset3
175484	4	410810	13	NULL	NULL	0	NULL	hypertrophic nail dystrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The main clinical features of the condition include painful and highly debilitating plantar keratoderma , hypertrophic nail dystrophy , oral leukokeratosis , and a variety of epidermal cysts .
	manualset3
175485	5	410810	13	NULL	NULL	0	NULL	oral leukokeratosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The main clinical features of the condition include painful and highly debilitating plantar keratoderma , hypertrophic nail dystrophy , oral leukokeratosis , and a variety of epidermal cysts .
	manualset3
175486	6	410810	13	NULL	NULL	0	NULL	variety of epidermal cysts 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The main clinical features of the condition include painful and highly debilitating plantar keratoderma , hypertrophic nail dystrophy , oral leukokeratosis , and a variety of epidermal cysts .
	manualset3
175487	1	410811	13	NULL	NULL	0	NULL	main effectors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The main effectors of flow regulation , the arterioles and small arteries , are located at a distance from the regions of tissue that they supply .
	manualset3
175488	2	410811	13	NULL	NULL	0	NULL	flow regulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The main effectors of flow regulation , the arterioles and small arteries , are located at a distance from the regions of tissue that they supply .
	manualset3
175489	3	410811	13	NULL	NULL	0	NULL	arterioles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The main effectors of flow regulation , the arterioles and small arteries , are located at a distance from the regions of tissue that they supply .
	manualset3
175490	4	410811	13	NULL	NULL	0	NULL	small arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The main effectors of flow regulation , the arterioles and small arteries , are located at a distance from the regions of tissue that they supply .
	manualset3
175491	5	410811	13	NULL	NULL	0	NULL	distance	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The main effectors of flow regulation , the arterioles and small arteries , are located at a distance from the regions of tissue that they supply .
	manualset3
175492	6	410811	13	NULL	NULL	0	NULL	 regions of tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The main effectors of flow regulation , the arterioles and small arteries , are located at a distance from the regions of tissue that they supply .
	manualset3
175493	1	410812	13	NULL	NULL	0	NULL	main features 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The main features of the IA sorbent were studied , such as the amount of hydrazide groups and antibodies attached onto oxidized diol silica particles .
	manualset3
175494	2	410812	13	NULL	NULL	0	NULL	IA sorbent 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The main features of the IA sorbent were studied , such as the amount of hydrazide groups and antibodies attached onto oxidized diol silica particles .
	manualset3
175495	3	410812	13	NULL	NULL	0	NULL	amount	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The main features of the IA sorbent were studied , such as the amount of hydrazide groups and antibodies attached onto oxidized diol silica particles .
	manualset3
175496	4	410812	13	NULL	NULL	0	NULL	hydrazide groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The main features of the IA sorbent were studied , such as the amount of hydrazide groups and antibodies attached onto oxidized diol silica particles .
	manualset3
175497	5	410812	13	NULL	NULL	0	NULL	antibodies 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The main features of the IA sorbent were studied , such as the amount of hydrazide groups and antibodies attached onto oxidized diol silica particles .
	manualset3
175498	6	410812	13	NULL	NULL	0	NULL	oxidized diol silica particles 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The main features of the IA sorbent were studied , such as the amount of hydrazide groups and antibodies attached onto oxidized diol silica particles .
	manualset3
175499	1	410813	13	NULL	NULL	NULL	NULL	main finding	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The main finding was that the susceptibilities of fluconazole-resistant C. albicans , C. dubliniensis , and Candida non-albicans to Mexican oregano , oregano , thyme , and ginger essential oils were higher than those of the fluconazole-susceptible yeasts ( P & lt ; 0.05 ) .
	manualset3
175500	2	410813	13	NULL	NULL	0	NULL	susceptibilities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The main finding was that the susceptibilities of fluconazole-resistant C. albicans , C. dubliniensis , and Candida non-albicans to Mexican oregano , oregano , thyme , and ginger essential oils were higher than those of the fluconazole-susceptible yeasts ( P & lt ; 0.05 ) .
	manualset3
175501	3	410813	13	NULL	NULL	0	NULL	fluconazole-resistant C. albicans 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The main finding was that the susceptibilities of fluconazole-resistant C. albicans , C. dubliniensis , and Candida non-albicans to Mexican oregano , oregano , thyme , and ginger essential oils were higher than those of the fluconazole-susceptible yeasts ( P & lt ; 0.05 ) .
	manualset3
175502	4	410813	13	NULL	NULL	0	NULL	C. dubliniensis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The main finding was that the susceptibilities of fluconazole-resistant C. albicans , C. dubliniensis , and Candida non-albicans to Mexican oregano , oregano , thyme , and ginger essential oils were higher than those of the fluconazole-susceptible yeasts ( P & lt ; 0.05 ) .
	manualset3
175503	5	410813	13	NULL	NULL	0	NULL	Candida non-albicans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The main finding was that the susceptibilities of fluconazole-resistant C. albicans , C. dubliniensis , and Candida non-albicans to Mexican oregano , oregano , thyme , and ginger essential oils were higher than those of the fluconazole-susceptible yeasts ( P & lt ; 0.05 ) .
	manualset3
175504	6	410813	13	NULL	NULL	0	NULL	Mexican oregano essential oil	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The main finding was that the susceptibilities of fluconazole-resistant C. albicans , C. dubliniensis , and Candida non-albicans to Mexican oregano , oregano , thyme , and ginger essential oils were higher than those of the fluconazole-susceptible yeasts ( P & lt ; 0.05 ) .
	manualset3
175505	7	410813	13	NULL	NULL	0	NULL	oregano essential oil	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The main finding was that the susceptibilities of fluconazole-resistant C. albicans , C. dubliniensis , and Candida non-albicans to Mexican oregano , oregano , thyme , and ginger essential oils were higher than those of the fluconazole-susceptible yeasts ( P & lt ; 0.05 ) .
	manualset3
175506	8	410813	13	NULL	NULL	0	NULL	thyme essential oil	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The main finding was that the susceptibilities of fluconazole-resistant C. albicans , C. dubliniensis , and Candida non-albicans to Mexican oregano , oregano , thyme , and ginger essential oils were higher than those of the fluconazole-susceptible yeasts ( P & lt ; 0.05 ) .
	manualset3
175507	9	410813	13	NULL	NULL	0	NULL	ginger essential oil	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The main finding was that the susceptibilities of fluconazole-resistant C. albicans , C. dubliniensis , and Candida non-albicans to Mexican oregano , oregano , thyme , and ginger essential oils were higher than those of the fluconazole-susceptible yeasts ( P & lt ; 0.05 ) .
	manualset3
175508	10	410813	13	NULL	NULL	0	NULL	fluconazole-susceptible yeasts	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The main finding was that the susceptibilities of fluconazole-resistant C. albicans , C. dubliniensis , and Candida non-albicans to Mexican oregano , oregano , thyme , and ginger essential oils were higher than those of the fluconazole-susceptible yeasts ( P & lt ; 0.05 ) .
	manualset3
175509	11	410813	13	NULL	NULL	0	NULL	P & lt ; 0.05	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The main finding was that the susceptibilities of fluconazole-resistant C. albicans , C. dubliniensis , and Candida non-albicans to Mexican oregano , oregano , thyme , and ginger essential oils were higher than those of the fluconazole-susceptible yeasts ( P & lt ; 0.05 ) .
	manualset3
175510	1	410814	13	NULL	NULL	0	NULL	total 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 871 persons reported at least one symptom of stress .
	manualset3
175511	2	410814	13	NULL	NULL	0	NULL	871 persons	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 871 persons reported at least one symptom of stress .
	manualset3
175512	3	410814	13	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 871 persons reported at least one symptom of stress .
	manualset3
175513	4	410814	13	NULL	NULL	0	NULL	symptom of stress 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 871 persons reported at least one symptom of stress .
	manualset3
175514	1	410815	13	NULL	NULL	NULL	NULL	main goal 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The main goal of the study was to evaluate the influence of the electrode orientation on the distribution of electric field in the tumor and surrounding tissue during electrochemotherapy .
	manualset3
175515	2	410815	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The main goal of the study was to evaluate the influence of the electrode orientation on the distribution of electric field in the tumor and surrounding tissue during electrochemotherapy .
	manualset3
175516	3	410815	13	NULL	NULL	0	NULL	influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The main goal of the study was to evaluate the influence of the electrode orientation on the distribution of electric field in the tumor and surrounding tissue during electrochemotherapy .
	manualset3
175517	4	410815	13	NULL	NULL	0	NULL	electrode orientation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The main goal of the study was to evaluate the influence of the electrode orientation on the distribution of electric field in the tumor and surrounding tissue during electrochemotherapy .
	manualset3
175518	5	410815	13	NULL	NULL	0	NULL	 distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The main goal of the study was to evaluate the influence of the electrode orientation on the distribution of electric field in the tumor and surrounding tissue during electrochemotherapy .
	manualset3
175519	6	410815	13	NULL	NULL	0	NULL	electric field	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The main goal of the study was to evaluate the influence of the electrode orientation on the distribution of electric field in the tumor and surrounding tissue during electrochemotherapy .
	manualset3
175520	7	410815	13	NULL	NULL	0	NULL	tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The main goal of the study was to evaluate the influence of the electrode orientation on the distribution of electric field in the tumor and surrounding tissue during electrochemotherapy .
	manualset3
175521	8	410815	13	NULL	NULL	0	NULL	 tissue 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The main goal of the study was to evaluate the influence of the electrode orientation on the distribution of electric field in the tumor and surrounding tissue during electrochemotherapy .
	manualset3
175522	9	410815	13	NULL	NULL	0	NULL	electrochemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The main goal of the study was to evaluate the influence of the electrode orientation on the distribution of electric field in the tumor and surrounding tissue during electrochemotherapy .
	manualset3
175523	1	410816	13	NULL	NULL	0	NULL	main interventions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The main interventions designed to reduce maternal obesity and GDM and their ability to break the vicious circle that perpetuates the transmission of obesity and metabolic conditions to the next generations are also addressed .
	manualset3
175524	2	410816	13	NULL	NULL	0	NULL	maternal obesity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The main interventions designed to reduce maternal obesity and GDM and their ability to break the vicious circle that perpetuates the transmission of obesity and metabolic conditions to the next generations are also addressed .
	manualset3
175525	3	410816	13	NULL	NULL	0	NULL	GDM	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The main interventions designed to reduce maternal obesity and GDM and their ability to break the vicious circle that perpetuates the transmission of obesity and metabolic conditions to the next generations are also addressed .
	manualset3
175526	4	410816	13	NULL	NULL	0	NULL	 ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The main interventions designed to reduce maternal obesity and GDM and their ability to break the vicious circle that perpetuates the transmission of obesity and metabolic conditions to the next generations are also addressed .
	manualset3
175527	5	410816	13	NULL	NULL	0	NULL	vicious circle	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The main interventions designed to reduce maternal obesity and GDM and their ability to break the vicious circle that perpetuates the transmission of obesity and metabolic conditions to the next generations are also addressed .
	manualset3
175528	6	410816	13	NULL	NULL	0	NULL	 transmission	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The main interventions designed to reduce maternal obesity and GDM and their ability to break the vicious circle that perpetuates the transmission of obesity and metabolic conditions to the next generations are also addressed .
	manualset3
175529	7	410816	13	NULL	NULL	0	NULL	obesity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The main interventions designed to reduce maternal obesity and GDM and their ability to break the vicious circle that perpetuates the transmission of obesity and metabolic conditions to the next generations are also addressed .
	manualset3
175530	8	410816	13	NULL	NULL	0	NULL	metabolic conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The main interventions designed to reduce maternal obesity and GDM and their ability to break the vicious circle that perpetuates the transmission of obesity and metabolic conditions to the next generations are also addressed .
	manualset3
175531	9	410816	13	NULL	NULL	0	NULL	generations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The main interventions designed to reduce maternal obesity and GDM and their ability to break the vicious circle that perpetuates the transmission of obesity and metabolic conditions to the next generations are also addressed .
	manualset3
175532	1	410817	13	NULL	NULL	0	NULL	objective	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The main objective of FEST is to develop a framework of common understanding which will assist those wishing to set up a Telemedicine service by providing structured guidance to the information required for such an endeavor .
	manualset3
175533	2	410817	13	NULL	NULL	0	NULL	FEST	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The main objective of FEST is to develop a framework of common understanding which will assist those wishing to set up a Telemedicine service by providing structured guidance to the information required for such an endeavor .
	manualset3
175534	3	410817	13	NULL	NULL	0	NULL	framework	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The main objective of FEST is to develop a framework of common understanding which will assist those wishing to set up a Telemedicine service by providing structured guidance to the information required for such an endeavor .
	manualset3
175535	4	410817	13	NULL	NULL	0	NULL	understanding 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The main objective of FEST is to develop a framework of common understanding which will assist those wishing to set up a Telemedicine service by providing structured guidance to the information required for such an endeavor .
	manualset3
175536	5	410817	13	NULL	NULL	0	NULL	Telemedicine service	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The main objective of FEST is to develop a framework of common understanding which will assist those wishing to set up a Telemedicine service by providing structured guidance to the information required for such an endeavor .
	manualset3
175537	6	410817	13	NULL	NULL	0	NULL	structured guidance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The main objective of FEST is to develop a framework of common understanding which will assist those wishing to set up a Telemedicine service by providing structured guidance to the information required for such an endeavor .
	manualset3
175538	7	410817	13	NULL	NULL	NULL	NULL	information	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The main objective of FEST is to develop a framework of common understanding which will assist those wishing to set up a Telemedicine service by providing structured guidance to the information required for such an endeavor .
	manualset3
175539	8	410817	13	NULL	NULL	0	NULL	endeavor	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The main objective of FEST is to develop a framework of common understanding which will assist those wishing to set up a Telemedicine service by providing structured guidance to the information required for such an endeavor .
	manualset3
175540	1	410818	13	NULL	NULL	0	NULL	 main objective	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The main objective of this study is to illustrate how adaptation to linguistic limitations takes place in a specific activity and is affected by factors pertaining to the social activity or the individuals .
	manualset3
175541	2	410818	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The main objective of this study is to illustrate how adaptation to linguistic limitations takes place in a specific activity and is affected by factors pertaining to the social activity or the individuals .
	manualset3
175542	3	410818	13	NULL	NULL	0	NULL	adaptation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The main objective of this study is to illustrate how adaptation to linguistic limitations takes place in a specific activity and is affected by factors pertaining to the social activity or the individuals .
	manualset3
175543	4	410818	13	NULL	NULL	0	NULL	linguistic limitations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The main objective of this study is to illustrate how adaptation to linguistic limitations takes place in a specific activity and is affected by factors pertaining to the social activity or the individuals .
	manualset3
175544	5	410818	13	NULL	NULL	0	NULL	 specific activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The main objective of this study is to illustrate how adaptation to linguistic limitations takes place in a specific activity and is affected by factors pertaining to the social activity or the individuals .
	manualset3
175545	6	410818	13	NULL	NULL	0	NULL	factors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The main objective of this study is to illustrate how adaptation to linguistic limitations takes place in a specific activity and is affected by factors pertaining to the social activity or the individuals .
	manualset3
175546	7	410818	13	NULL	NULL	0	NULL	social activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The main objective of this study is to illustrate how adaptation to linguistic limitations takes place in a specific activity and is affected by factors pertaining to the social activity or the individuals .
	manualset3
175547	8	410818	13	NULL	NULL	0	NULL	individuals 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The main objective of this study is to illustrate how adaptation to linguistic limitations takes place in a specific activity and is affected by factors pertaining to the social activity or the individuals .
	manualset3
175548	1	410819	13	NULL	NULL	0	NULL	main objectives	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The main objectives of this study were to ( 1 ) clarify the factors affecting the ability and efficiency of PCP biodegradation by P. mendocina NSYSU , and ( 2 ) optimize the use of this bacterium in bioremediation of PCP .
	manualset3
175549	2	410819	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The main objectives of this study were to ( 1 ) clarify the factors affecting the ability and efficiency of PCP biodegradation by P. mendocina NSYSU , and ( 2 ) optimize the use of this bacterium in bioremediation of PCP .
	manualset3
175550	3	410819	13	NULL	NULL	0	NULL	 factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The main objectives of this study were to ( 1 ) clarify the factors affecting the ability and efficiency of PCP biodegradation by P. mendocina NSYSU , and ( 2 ) optimize the use of this bacterium in bioremediation of PCP .
	manualset3
175551	4	410819	13	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The main objectives of this study were to ( 1 ) clarify the factors affecting the ability and efficiency of PCP biodegradation by P. mendocina NSYSU , and ( 2 ) optimize the use of this bacterium in bioremediation of PCP .
	manualset3
175552	5	410819	13	NULL	NULL	0	NULL	efficiency	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The main objectives of this study were to ( 1 ) clarify the factors affecting the ability and efficiency of PCP biodegradation by P. mendocina NSYSU , and ( 2 ) optimize the use of this bacterium in bioremediation of PCP .
	manualset3
175553	6	410819	13	NULL	NULL	0	NULL	PCP biodegradation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The main objectives of this study were to ( 1 ) clarify the factors affecting the ability and efficiency of PCP biodegradation by P. mendocina NSYSU , and ( 2 ) optimize the use of this bacterium in bioremediation of PCP .
	manualset3
175554	7	410819	13	NULL	NULL	0	NULL	P. mendocina NSYSU	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The main objectives of this study were to ( 1 ) clarify the factors affecting the ability and efficiency of PCP biodegradation by P. mendocina NSYSU , and ( 2 ) optimize the use of this bacterium in bioremediation of PCP .
	manualset3
175555	8	410819	13	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The main objectives of this study were to ( 1 ) clarify the factors affecting the ability and efficiency of PCP biodegradation by P. mendocina NSYSU , and ( 2 ) optimize the use of this bacterium in bioremediation of PCP .
	manualset3
175556	9	410819	13	NULL	NULL	0	NULL	bacterium 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The main objectives of this study were to ( 1 ) clarify the factors affecting the ability and efficiency of PCP biodegradation by P. mendocina NSYSU , and ( 2 ) optimize the use of this bacterium in bioremediation of PCP .
	manualset3
175557	10	410819	13	NULL	NULL	0	NULL	bioremediation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The main objectives of this study were to ( 1 ) clarify the factors affecting the ability and efficiency of PCP biodegradation by P. mendocina NSYSU , and ( 2 ) optimize the use of this bacterium in bioremediation of PCP .
	manualset3
175558	11	410819	13	NULL	NULL	0	NULL	PCP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The main objectives of this study were to ( 1 ) clarify the factors affecting the ability and efficiency of PCP biodegradation by P. mendocina NSYSU , and ( 2 ) optimize the use of this bacterium in bioremediation of PCP .
	manualset3
175559	1	410820	13	NULL	NULL	0	NULL	pathogene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The main pathogene of sepsis at present is staphylococcus .
	manualset3
175560	2	410820	13	NULL	NULL	0	NULL	sepsis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The main pathogene of sepsis at present is staphylococcus .
	manualset3
175561	3	410820	13	NULL	NULL	0	NULL	present	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The main pathogene of sepsis at present is staphylococcus .
	manualset3
175562	4	410820	13	NULL	NULL	0	NULL	staphylococcus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The main pathogene of sepsis at present is staphylococcus .
	manualset3
175563	1	410821	13	NULL	NULL	0	NULL	problem	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The main problem associated with this approach is the source of electricity .
	manualset3
175564	2	410821	13	NULL	NULL	0	NULL	approach	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The main problem associated with this approach is the source of electricity .
	manualset3
175565	3	410821	13	NULL	NULL	0	NULL	source 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The main problem associated with this approach is the source of electricity .
	manualset3
175566	4	410821	13	NULL	NULL	0	NULL	 electricity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The main problem associated with this approach is the source of electricity .
	manualset3
175567	1	410822	13	NULL	NULL	NULL	NULL	problem	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The main problem with these compounds , however , is formulation stability : Alprenoxime has a t90 of only 2-3 months .
	manualset3
175568	2	410822	13	NULL	NULL	0	NULL	compounds 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The main problem with these compounds , however , is formulation stability : Alprenoxime has a t90 of only 2-3 months .
	manualset3
175569	3	410822	13	NULL	NULL	0	NULL	formulation stability	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The main problem with these compounds , however , is formulation stability : Alprenoxime has a t90 of only 2-3 months .
	manualset3
175570	4	410822	13	NULL	NULL	0	NULL	Alprenoxime	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The main problem with these compounds , however , is formulation stability : Alprenoxime has a t90 of only 2-3 months .
	manualset3
175571	5	410822	13	NULL	NULL	0	NULL	t90 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The main problem with these compounds , however , is formulation stability : Alprenoxime has a t90 of only 2-3 months .
	manualset3
175572	6	410822	13	NULL	NULL	0	NULL	2-3 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The main problem with these compounds , however , is formulation stability : Alprenoxime has a t90 of only 2-3 months .
	manualset3
175573	1	410823	13	NULL	NULL	0	NULL	serious risks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The main serious risks of anastomotic construction in the colon and rectum include dehiscence and stricture formation .
	manualset3
175574	2	410823	13	NULL	NULL	0	NULL	anastomotic construction	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The main serious risks of anastomotic construction in the colon and rectum include dehiscence and stricture formation .
	manualset3
175575	3	410823	13	NULL	NULL	0	NULL	colon	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The main serious risks of anastomotic construction in the colon and rectum include dehiscence and stricture formation .
	manualset3
175576	4	410823	13	NULL	NULL	0	NULL	rectum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The main serious risks of anastomotic construction in the colon and rectum include dehiscence and stricture formation .
	manualset3
175577	5	410823	13	NULL	NULL	0	NULL	dehiscence 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The main serious risks of anastomotic construction in the colon and rectum include dehiscence and stricture formation .
	manualset3
175578	6	410823	13	NULL	NULL	0	NULL	stricture formation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The main serious risks of anastomotic construction in the colon and rectum include dehiscence and stricture formation .
	manualset3
175579	1	410824	13	NULL	NULL	0	NULL	maintenance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The maintenance of metabolic activity in the paraventricular nucleus of vasopressin-treated Brattleboro rats suggests that this structure contributes importantly to the metabolism of neural lobe .
	manualset3
175580	2	410824	13	NULL	NULL	0	NULL	metabolic activity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The maintenance of metabolic activity in the paraventricular nucleus of vasopressin-treated Brattleboro rats suggests that this structure contributes importantly to the metabolism of neural lobe .
	manualset3
175581	3	410824	13	NULL	NULL	0	NULL	paraventricular nucleus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The maintenance of metabolic activity in the paraventricular nucleus of vasopressin-treated Brattleboro rats suggests that this structure contributes importantly to the metabolism of neural lobe .
	manualset3
175582	4	410824	13	NULL	NULL	0	NULL	vasopressin-treated Brattleboro rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The maintenance of metabolic activity in the paraventricular nucleus of vasopressin-treated Brattleboro rats suggests that this structure contributes importantly to the metabolism of neural lobe .
	manualset3
175583	5	410824	13	NULL	NULL	0	NULL	structure 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The maintenance of metabolic activity in the paraventricular nucleus of vasopressin-treated Brattleboro rats suggests that this structure contributes importantly to the metabolism of neural lobe .
	manualset3
175584	6	410824	13	NULL	NULL	0	NULL	metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The maintenance of metabolic activity in the paraventricular nucleus of vasopressin-treated Brattleboro rats suggests that this structure contributes importantly to the metabolism of neural lobe .
	manualset3
175585	7	410824	13	NULL	NULL	0	NULL	neural lobe	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The maintenance of metabolic activity in the paraventricular nucleus of vasopressin-treated Brattleboro rats suggests that this structure contributes importantly to the metabolism of neural lobe .
	manualset3
175586	1	410825	13	NULL	NULL	0	NULL	major FAs 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The major FAs that characterized the tested strain were C16 : 0 , C18 : 1 , C18 : 2 , C18 : 3 and C18 : 0 .
	manualset3
175587	2	410825	13	NULL	NULL	0	NULL	strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The major FAs that characterized the tested strain were C16 : 0 , C18 : 1 , C18 : 2 , C18 : 3 and C18 : 0 .
	manualset3
175588	3	410825	13	NULL	NULL	0	NULL	C16 : 0	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The major FAs that characterized the tested strain were C16 : 0 , C18 : 1 , C18 : 2 , C18 : 3 and C18 : 0 .
	manualset3
175589	4	410825	13	NULL	NULL	0	NULL	C18 : 1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The major FAs that characterized the tested strain were C16 : 0 , C18 : 1 , C18 : 2 , C18 : 3 and C18 : 0 .
	manualset3
175590	5	410825	13	NULL	NULL	0	NULL	C18 : 2 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The major FAs that characterized the tested strain were C16 : 0 , C18 : 1 , C18 : 2 , C18 : 3 and C18 : 0 .
	manualset3
175591	6	410825	13	NULL	NULL	0	NULL	C18 : 3 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The major FAs that characterized the tested strain were C16 : 0 , C18 : 1 , C18 : 2 , C18 : 3 and C18 : 0 .
	manualset3
175592	7	410825	13	NULL	NULL	0	NULL	C18 : 0	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The major FAs that characterized the tested strain were C16 : 0 , C18 : 1 , C18 : 2 , C18 : 3 and C18 : 0 .
	manualset3
175594	2	410826	13	NULL	NULL	0	NULL	MR imaging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The major advantage of MR imaging over computed tomography or angiography is the exquisite difference in contrast between hemangiomas and the surrounding structures on T2-weighted MR images , in which hemangiomas have a relatively intense signal .
	manualset3
175595	3	410826	13	NULL	NULL	0	NULL	computed tomography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The major advantage of MR imaging over computed tomography or angiography is the exquisite difference in contrast between hemangiomas and the surrounding structures on T2-weighted MR images , in which hemangiomas have a relatively intense signal .
	manualset3
175596	4	410826	13	NULL	NULL	0	NULL	angiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The major advantage of MR imaging over computed tomography or angiography is the exquisite difference in contrast between hemangiomas and the surrounding structures on T2-weighted MR images , in which hemangiomas have a relatively intense signal .
	manualset3
175597	5	410826	13	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The major advantage of MR imaging over computed tomography or angiography is the exquisite difference in contrast between hemangiomas and the surrounding structures on T2-weighted MR images , in which hemangiomas have a relatively intense signal .
	manualset3
175598	6	410826	13	NULL	NULL	0	NULL	contrast	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The major advantage of MR imaging over computed tomography or angiography is the exquisite difference in contrast between hemangiomas and the surrounding structures on T2-weighted MR images , in which hemangiomas have a relatively intense signal .
	manualset3
175599	7	410826	13	NULL	NULL	0	NULL	hemangiomas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The major advantage of MR imaging over computed tomography or angiography is the exquisite difference in contrast between hemangiomas and the surrounding structures on T2-weighted MR images , in which hemangiomas have a relatively intense signal .
	manualset3
175600	8	410826	13	NULL	NULL	0	NULL	structures	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The major advantage of MR imaging over computed tomography or angiography is the exquisite difference in contrast between hemangiomas and the surrounding structures on T2-weighted MR images , in which hemangiomas have a relatively intense signal .
	manualset3
175601	9	410826	13	NULL	NULL	0	NULL	T2-weighted MR images 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The major advantage of MR imaging over computed tomography or angiography is the exquisite difference in contrast between hemangiomas and the surrounding structures on T2-weighted MR images , in which hemangiomas have a relatively intense signal .
	manualset3
175602	10	410826	13	NULL	NULL	0	NULL	hemangiomas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The major advantage of MR imaging over computed tomography or angiography is the exquisite difference in contrast between hemangiomas and the surrounding structures on T2-weighted MR images , in which hemangiomas have a relatively intense signal .
	manualset3
175603	11	410826	13	NULL	NULL	0	NULL	intense signal	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The major advantage of MR imaging over computed tomography or angiography is the exquisite difference in contrast between hemangiomas and the surrounding structures on T2-weighted MR images , in which hemangiomas have a relatively intense signal .
	manualset3
175593	1	410827	13	NULL	NULL	NULL	NULL	major biotransformation pathways	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The major biotransformation pathways are carbonyl reduction , O-methylation at C-3 ' , O-methylation after aromatic hydroxylation at the position C-2 ' on phenyl B ring and O-demethylation on A ring .
	manualset3
175604	2	410827	13	NULL	NULL	0	NULL	carbonyl reduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The major biotransformation pathways are carbonyl reduction , O-methylation at C-3 ' , O-methylation after aromatic hydroxylation at the position C-2 ' on phenyl B ring and O-demethylation on A ring .
	manualset3
175605	3	410827	13	NULL	NULL	0	NULL	O-methylation at C-3 '	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The major biotransformation pathways are carbonyl reduction , O-methylation at C-3 ' , O-methylation after aromatic hydroxylation at the position C-2 ' on phenyl B ring and O-demethylation on A ring .
	manualset3
175606	4	410827	13	NULL	NULL	0	NULL	O-methylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The major biotransformation pathways are carbonyl reduction , O-methylation at C-3 ' , O-methylation after aromatic hydroxylation at the position C-2 ' on phenyl B ring and O-demethylation on A ring .
	manualset3
175607	5	410827	13	NULL	NULL	0	NULL	aromatic hydroxylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The major biotransformation pathways are carbonyl reduction , O-methylation at C-3 ' , O-methylation after aromatic hydroxylation at the position C-2 ' on phenyl B ring and O-demethylation on A ring .
	manualset3
175608	6	410827	13	NULL	NULL	0	NULL	position C-2 ' on phenyl B ring 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The major biotransformation pathways are carbonyl reduction , O-methylation at C-3 ' , O-methylation after aromatic hydroxylation at the position C-2 ' on phenyl B ring and O-demethylation on A ring .
	manualset3
175609	7	410827	13	NULL	NULL	0	NULL	O-demethylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The major biotransformation pathways are carbonyl reduction , O-methylation at C-3 ' , O-methylation after aromatic hydroxylation at the position C-2 ' on phenyl B ring and O-demethylation on A ring .
	manualset3
175610	8	410827	13	NULL	NULL	0	NULL	 A ring	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The major biotransformation pathways are carbonyl reduction , O-methylation at C-3 ' , O-methylation after aromatic hydroxylation at the position C-2 ' on phenyl B ring and O-demethylation on A ring .
	manualset3
175611	1	410828	13	NULL	NULL	0	NULL	major causes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The major causes of death not related to AIDS in hemophiliacs were bleeding , liver cirrhosis , and liver cancer .
	manualset3
175612	2	410828	13	NULL	NULL	0	NULL	death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The major causes of death not related to AIDS in hemophiliacs were bleeding , liver cirrhosis , and liver cancer .
	manualset3
175613	3	410828	13	NULL	NULL	0	NULL	AIDS 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The major causes of death not related to AIDS in hemophiliacs were bleeding , liver cirrhosis , and liver cancer .
	manualset3
175614	4	410828	13	NULL	NULL	0	NULL	hemophiliacs	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The major causes of death not related to AIDS in hemophiliacs were bleeding , liver cirrhosis , and liver cancer .
	manualset3
175615	5	410828	13	NULL	NULL	0	NULL	liver cirrhosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The major causes of death not related to AIDS in hemophiliacs were bleeding , liver cirrhosis , and liver cancer .
	manualset3
175616	6	410828	13	NULL	NULL	0	NULL	liver cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The major causes of death not related to AIDS in hemophiliacs were bleeding , liver cirrhosis , and liver cancer .
	manualset3
175617	1	410829	13	NULL	NULL	0	NULL	major class	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The major class of atrial natriuretic peptide ( ANP ) receptors was isolated from cultured vascular smooth muscle cells , and a partial amino acid sequence was obtained .
	manualset3
175618	2	410829	13	NULL	NULL	0	NULL	 atrial natriuretic peptide ( ANP ) receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The major class of atrial natriuretic peptide ( ANP ) receptors was isolated from cultured vascular smooth muscle cells , and a partial amino acid sequence was obtained .
	manualset3
175619	3	410829	13	NULL	NULL	0	NULL	cultured vascular smooth muscle cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The major class of atrial natriuretic peptide ( ANP ) receptors was isolated from cultured vascular smooth muscle cells , and a partial amino acid sequence was obtained .
	manualset3
175620	4	410829	13	NULL	NULL	0	NULL	partial amino acid sequence	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The major class of atrial natriuretic peptide ( ANP ) receptors was isolated from cultured vascular smooth muscle cells , and a partial amino acid sequence was obtained .
	manualset3
175621	1	410830	13	NULL	NULL	0	NULL	major components 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The major components of rose water volatiles obtained from the bud , half bloom and full bloom stages of cultivar ` Ranisahiba ' were phenyl ethyl alcohol ( 66.2-79 .0 % ) , geraniol ( 3.3-6 .6 % ) and citronellol ( 1.8-5 .5 % ) .
	manualset3
175622	2	410830	13	NULL	NULL	0	NULL	rose water volatiles 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The major components of rose water volatiles obtained from the bud , half bloom and full bloom stages of cultivar ` Ranisahiba ' were phenyl ethyl alcohol ( 66.2-79 .0 % ) , geraniol ( 3.3-6 .6 % ) and citronellol ( 1.8-5 .5 % ) .
	manualset3
175623	3	410830	13	NULL	NULL	0	NULL	bud stage	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The major components of rose water volatiles obtained from the bud , half bloom and full bloom stages of cultivar ` Ranisahiba ' were phenyl ethyl alcohol ( 66.2-79 .0 % ) , geraniol ( 3.3-6 .6 % ) and citronellol ( 1.8-5 .5 % ) .
	manualset3
175624	4	410830	13	NULL	NULL	0	NULL	half bloom stage	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The major components of rose water volatiles obtained from the bud , half bloom and full bloom stages of cultivar ` Ranisahiba ' were phenyl ethyl alcohol ( 66.2-79 .0 % ) , geraniol ( 3.3-6 .6 % ) and citronellol ( 1.8-5 .5 % ) .
	manualset3
175625	5	410830	13	NULL	NULL	0	NULL	full bloom stage	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The major components of rose water volatiles obtained from the bud , half bloom and full bloom stages of cultivar ` Ranisahiba ' were phenyl ethyl alcohol ( 66.2-79 .0 % ) , geraniol ( 3.3-6 .6 % ) and citronellol ( 1.8-5 .5 % ) .
	manualset3
175626	6	410830	13	NULL	NULL	0	NULL	cultivar	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The major components of rose water volatiles obtained from the bud , half bloom and full bloom stages of cultivar ` Ranisahiba ' were phenyl ethyl alcohol ( 66.2-79 .0 % ) , geraniol ( 3.3-6 .6 % ) and citronellol ( 1.8-5 .5 % ) .
	manualset3
175627	7	410830	13	NULL	NULL	0	NULL	Ranisahiba	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The major components of rose water volatiles obtained from the bud , half bloom and full bloom stages of cultivar ` Ranisahiba ' were phenyl ethyl alcohol ( 66.2-79 .0 % ) , geraniol ( 3.3-6 .6 % ) and citronellol ( 1.8-5 .5 % ) .
	manualset3
175628	8	410830	13	NULL	NULL	0	NULL	phenyl ethyl alcohol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The major components of rose water volatiles obtained from the bud , half bloom and full bloom stages of cultivar ` Ranisahiba ' were phenyl ethyl alcohol ( 66.2-79 .0 % ) , geraniol ( 3.3-6 .6 % ) and citronellol ( 1.8-5 .5 % ) .
	manualset3
175629	9	410830	13	NULL	NULL	0	NULL	66.2-79 .0 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The major components of rose water volatiles obtained from the bud , half bloom and full bloom stages of cultivar ` Ranisahiba ' were phenyl ethyl alcohol ( 66.2-79 .0 % ) , geraniol ( 3.3-6 .6 % ) and citronellol ( 1.8-5 .5 % ) .
	manualset3
175630	10	410830	13	NULL	NULL	0	NULL	geraniol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The major components of rose water volatiles obtained from the bud , half bloom and full bloom stages of cultivar ` Ranisahiba ' were phenyl ethyl alcohol ( 66.2-79 .0 % ) , geraniol ( 3.3-6 .6 % ) and citronellol ( 1.8-5 .5 % ) .
	manualset3
175631	11	410830	13	NULL	NULL	0	NULL	3.3-6 .6 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The major components of rose water volatiles obtained from the bud , half bloom and full bloom stages of cultivar ` Ranisahiba ' were phenyl ethyl alcohol ( 66.2-79 .0 % ) , geraniol ( 3.3-6 .6 % ) and citronellol ( 1.8-5 .5 % ) .
	manualset3
175632	12	410830	13	NULL	NULL	0	NULL	citronellol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The major components of rose water volatiles obtained from the bud , half bloom and full bloom stages of cultivar ` Ranisahiba ' were phenyl ethyl alcohol ( 66.2-79 .0 % ) , geraniol ( 3.3-6 .6 % ) and citronellol ( 1.8-5 .5 % ) .
	manualset3
175633	13	410830	13	NULL	NULL	0	NULL	1.8-5 .5 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The major components of rose water volatiles obtained from the bud , half bloom and full bloom stages of cultivar ` Ranisahiba ' were phenyl ethyl alcohol ( 66.2-79 .0 % ) , geraniol ( 3.3-6 .6 % ) and citronellol ( 1.8-5 .5 % ) .
	manualset3
175675	1	410831	13	NULL	NULL	0	NULL	total 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 93 polypeptides were found to be candidates for differential distribution with a nominal p-value & lt ; 0.05 , though these differences did not reach significance when multiple testing was accounted for .
	manualset3
175676	2	410831	13	NULL	NULL	0	NULL	93 polypeptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 93 polypeptides were found to be candidates for differential distribution with a nominal p-value & lt ; 0.05 , though these differences did not reach significance when multiple testing was accounted for .
	manualset3
175692	3	410831	13	NULL	NULL	0	NULL	candidates	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 93 polypeptides were found to be candidates for differential distribution with a nominal p-value & lt ; 0.05 , though these differences did not reach significance when multiple testing was accounted for .
	manualset3
175693	4	410831	13	NULL	NULL	0	NULL	distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 93 polypeptides were found to be candidates for differential distribution with a nominal p-value & lt ; 0.05 , though these differences did not reach significance when multiple testing was accounted for .
	manualset3
175694	5	410831	13	NULL	NULL	0	NULL	p-value 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 93 polypeptides were found to be candidates for differential distribution with a nominal p-value & lt ; 0.05 , though these differences did not reach significance when multiple testing was accounted for .
	manualset3
175695	6	410831	13	NULL	NULL	0	NULL	0.05 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 93 polypeptides were found to be candidates for differential distribution with a nominal p-value & lt ; 0.05 , though these differences did not reach significance when multiple testing was accounted for .
	manualset3
175696	7	410831	13	NULL	NULL	0	NULL	differences	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 93 polypeptides were found to be candidates for differential distribution with a nominal p-value & lt ; 0.05 , though these differences did not reach significance when multiple testing was accounted for .
	manualset3
175697	8	410831	13	NULL	NULL	0	NULL	significance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 93 polypeptides were found to be candidates for differential distribution with a nominal p-value & lt ; 0.05 , though these differences did not reach significance when multiple testing was accounted for .
	manualset3
175698	9	410831	13	NULL	NULL	0	NULL	multiple testing 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 93 polypeptides were found to be candidates for differential distribution with a nominal p-value & lt ; 0.05 , though these differences did not reach significance when multiple testing was accounted for .
	manualset3
175699	1	410832	13	NULL	NULL	0	NULL	major components 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The major components of this framework are the designs of union action and evolving rate .
	manualset3
175700	2	410832	13	NULL	NULL	0	NULL	framework 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The major components of this framework are the designs of union action and evolving rate .
	manualset3
175701	3	410832	13	NULL	NULL	0	NULL	designs	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The major components of this framework are the designs of union action and evolving rate .
	manualset3
175702	4	410832	13	NULL	NULL	0	NULL	union action	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The major components of this framework are the designs of union action and evolving rate .
	manualset3
175703	5	410832	13	NULL	NULL	0	NULL	rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The major components of this framework are the designs of union action and evolving rate .
	manualset3
175704	1	410833	13	NULL	NULL	0	NULL	decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The major decrease in plasma volume was during the running stage of the triathlon during which it decreased by 6.2 % + / - 1.7 % , of which 3.0 % + / - 1.8 % was attributable to exercise alone .
	manualset3
175705	2	410833	13	NULL	NULL	0	NULL	plasma volume	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The major decrease in plasma volume was during the running stage of the triathlon during which it decreased by 6.2 % + / - 1.7 % , of which 3.0 % + / - 1.8 % was attributable to exercise alone .
	manualset3
175706	3	410833	13	NULL	NULL	0	NULL	running stage 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The major decrease in plasma volume was during the running stage of the triathlon during which it decreased by 6.2 % + / - 1.7 % , of which 3.0 % + / - 1.8 % was attributable to exercise alone .
	manualset3
175707	4	410833	13	NULL	NULL	0	NULL	 triathlon	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The major decrease in plasma volume was during the running stage of the triathlon during which it decreased by 6.2 % + / - 1.7 % , of which 3.0 % + / - 1.8 % was attributable to exercise alone .
	manualset3
175708	5	410833	13	NULL	NULL	0	NULL	6.2 % + / - 1.7 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The major decrease in plasma volume was during the running stage of the triathlon during which it decreased by 6.2 % + / - 1.7 % , of which 3.0 % + / - 1.8 % was attributable to exercise alone .
	manualset3
175709	6	410833	13	NULL	NULL	0	NULL	 3.0 % + / - 1.8 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The major decrease in plasma volume was during the running stage of the triathlon during which it decreased by 6.2 % + / - 1.7 % , of which 3.0 % + / - 1.8 % was attributable to exercise alone .
	manualset3
175710	1	410834	13	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The major difference between the two proteins is that the nucleating activity of cofilin-actin .
	manualset3
175711	2	410834	13	NULL	NULL	0	NULL	two proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The major difference between the two proteins is that the nucleating activity of cofilin-actin .
	manualset3
175712	3	410834	13	NULL	NULL	0	NULL	nucleating activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The major difference between the two proteins is that the nucleating activity of cofilin-actin .
	manualset3
175713	4	410834	13	NULL	NULL	0	NULL	cofilin-actin 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The major difference between the two proteins is that the nucleating activity of cofilin-actin .
	manualset3
175714	1	410835	13	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The major difference in the fatty acid composition of M. plumulosa cultured on silty sediment compared to amphipods cultured on a sand substrate and both fed Sera micron was an increase in the ratio of omega-3 to omega-6 PUFAs , indicating that the silty sediment provides additional food sources rich in omega-3 PUFAs .
	manualset3
175715	2	410835	13	NULL	NULL	0	NULL	fatty acid	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The major difference in the fatty acid composition of M. plumulosa cultured on silty sediment compared to amphipods cultured on a sand substrate and both fed Sera micron was an increase in the ratio of omega-3 to omega-6 PUFAs , indicating that the silty sediment provides additional food sources rich in omega-3 PUFAs .
	manualset3
175716	3	410835	13	NULL	NULL	0	NULL	composition	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The major difference in the fatty acid composition of M. plumulosa cultured on silty sediment compared to amphipods cultured on a sand substrate and both fed Sera micron was an increase in the ratio of omega-3 to omega-6 PUFAs , indicating that the silty sediment provides additional food sources rich in omega-3 PUFAs .
	manualset3
175717	4	410835	13	NULL	NULL	0	NULL	M. plumulosa	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The major difference in the fatty acid composition of M. plumulosa cultured on silty sediment compared to amphipods cultured on a sand substrate and both fed Sera micron was an increase in the ratio of omega-3 to omega-6 PUFAs , indicating that the silty sediment provides additional food sources rich in omega-3 PUFAs .
	manualset3
175718	5	410835	13	NULL	NULL	0	NULL	silty sediment	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The major difference in the fatty acid composition of M. plumulosa cultured on silty sediment compared to amphipods cultured on a sand substrate and both fed Sera micron was an increase in the ratio of omega-3 to omega-6 PUFAs , indicating that the silty sediment provides additional food sources rich in omega-3 PUFAs .
	manualset3
175719	6	410835	13	NULL	NULL	0	NULL	amphipods	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The major difference in the fatty acid composition of M. plumulosa cultured on silty sediment compared to amphipods cultured on a sand substrate and both fed Sera micron was an increase in the ratio of omega-3 to omega-6 PUFAs , indicating that the silty sediment provides additional food sources rich in omega-3 PUFAs .
	manualset3
175720	7	410835	13	NULL	NULL	0	NULL	sand substrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The major difference in the fatty acid composition of M. plumulosa cultured on silty sediment compared to amphipods cultured on a sand substrate and both fed Sera micron was an increase in the ratio of omega-3 to omega-6 PUFAs , indicating that the silty sediment provides additional food sources rich in omega-3 PUFAs .
	manualset3
175721	8	410835	13	NULL	NULL	0	NULL	Sera micron 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The major difference in the fatty acid composition of M. plumulosa cultured on silty sediment compared to amphipods cultured on a sand substrate and both fed Sera micron was an increase in the ratio of omega-3 to omega-6 PUFAs , indicating that the silty sediment provides additional food sources rich in omega-3 PUFAs .
	manualset3
175722	9	410835	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The major difference in the fatty acid composition of M. plumulosa cultured on silty sediment compared to amphipods cultured on a sand substrate and both fed Sera micron was an increase in the ratio of omega-3 to omega-6 PUFAs , indicating that the silty sediment provides additional food sources rich in omega-3 PUFAs .
	manualset3
175723	10	410835	13	NULL	NULL	0	NULL	ratio	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The major difference in the fatty acid composition of M. plumulosa cultured on silty sediment compared to amphipods cultured on a sand substrate and both fed Sera micron was an increase in the ratio of omega-3 to omega-6 PUFAs , indicating that the silty sediment provides additional food sources rich in omega-3 PUFAs .
	manualset3
175724	11	410835	13	NULL	NULL	0	NULL	omega-3	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The major difference in the fatty acid composition of M. plumulosa cultured on silty sediment compared to amphipods cultured on a sand substrate and both fed Sera micron was an increase in the ratio of omega-3 to omega-6 PUFAs , indicating that the silty sediment provides additional food sources rich in omega-3 PUFAs .
	manualset3
175725	12	410835	13	NULL	NULL	0	NULL	omega-6 PUFAs 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The major difference in the fatty acid composition of M. plumulosa cultured on silty sediment compared to amphipods cultured on a sand substrate and both fed Sera micron was an increase in the ratio of omega-3 to omega-6 PUFAs , indicating that the silty sediment provides additional food sources rich in omega-3 PUFAs .
	manualset3
175726	13	410835	13	NULL	NULL	0	NULL	 silty sediment	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The major difference in the fatty acid composition of M. plumulosa cultured on silty sediment compared to amphipods cultured on a sand substrate and both fed Sera micron was an increase in the ratio of omega-3 to omega-6 PUFAs , indicating that the silty sediment provides additional food sources rich in omega-3 PUFAs .
	manualset3
175727	14	410835	13	NULL	NULL	0	NULL	food sources	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The major difference in the fatty acid composition of M. plumulosa cultured on silty sediment compared to amphipods cultured on a sand substrate and both fed Sera micron was an increase in the ratio of omega-3 to omega-6 PUFAs , indicating that the silty sediment provides additional food sources rich in omega-3 PUFAs .
	manualset3
175728	15	410835	13	NULL	NULL	0	NULL	omega-3 PUFAs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The major difference in the fatty acid composition of M. plumulosa cultured on silty sediment compared to amphipods cultured on a sand substrate and both fed Sera micron was an increase in the ratio of omega-3 to omega-6 PUFAs , indicating that the silty sediment provides additional food sources rich in omega-3 PUFAs .
	manualset3
175736	1	410836	13	NULL	NULL	0	NULL	goal 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The major goal of transplantation immunology is to develop tolerance to allograft transplants and long-term drug-free survival .
	manualset3
175738	2	410836	13	NULL	NULL	0	NULL	transplantation immunology 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The major goal of transplantation immunology is to develop tolerance to allograft transplants and long-term drug-free survival .
	manualset3
175739	3	410836	13	NULL	NULL	0	NULL	tolerance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The major goal of transplantation immunology is to develop tolerance to allograft transplants and long-term drug-free survival .
	manualset3
175741	4	410836	13	NULL	NULL	0	NULL	allograft transplants 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The major goal of transplantation immunology is to develop tolerance to allograft transplants and long-term drug-free survival .
	manualset3
175744	5	410836	13	NULL	NULL	0	NULL	drug-free survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The major goal of transplantation immunology is to develop tolerance to allograft transplants and long-term drug-free survival .
	manualset3
175745	1	410837	13	NULL	NULL	0	NULL	objective	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The major objective of this model was to test an earlier conceptual model in which we proposed that clone size potential and sensitivity to gm-CSA are functional properties of granulocyte-macrophage progenitor cells , properties that gradually change as the cells differentiate down the granulocyte-monocyte pathway .
	manualset3
175746	2	410837	13	NULL	NULL	0	NULL	model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The major objective of this model was to test an earlier conceptual model in which we proposed that clone size potential and sensitivity to gm-CSA are functional properties of granulocyte-macrophage progenitor cells , properties that gradually change as the cells differentiate down the granulocyte-monocyte pathway .
	manualset3
175747	3	410837	13	NULL	NULL	0	NULL	conceptual model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The major objective of this model was to test an earlier conceptual model in which we proposed that clone size potential and sensitivity to gm-CSA are functional properties of granulocyte-macrophage progenitor cells , properties that gradually change as the cells differentiate down the granulocyte-monocyte pathway .
	manualset3
175748	4	410837	13	NULL	NULL	0	NULL	clone size	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The major objective of this model was to test an earlier conceptual model in which we proposed that clone size potential and sensitivity to gm-CSA are functional properties of granulocyte-macrophage progenitor cells , properties that gradually change as the cells differentiate down the granulocyte-monocyte pathway .
	manualset3
175749	5	410837	13	NULL	NULL	0	NULL	sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The major objective of this model was to test an earlier conceptual model in which we proposed that clone size potential and sensitivity to gm-CSA are functional properties of granulocyte-macrophage progenitor cells , properties that gradually change as the cells differentiate down the granulocyte-monocyte pathway .
	manualset3
175753	6	410837	13	NULL	NULL	0	NULL	gm-CSA 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The major objective of this model was to test an earlier conceptual model in which we proposed that clone size potential and sensitivity to gm-CSA are functional properties of granulocyte-macrophage progenitor cells , properties that gradually change as the cells differentiate down the granulocyte-monocyte pathway .
	manualset3
175755	7	410837	13	NULL	NULL	0	NULL	functional properties	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The major objective of this model was to test an earlier conceptual model in which we proposed that clone size potential and sensitivity to gm-CSA are functional properties of granulocyte-macrophage progenitor cells , properties that gradually change as the cells differentiate down the granulocyte-monocyte pathway .
	manualset3
175756	8	410837	13	NULL	NULL	0	NULL	granulocyte-macrophage progenitor cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The major objective of this model was to test an earlier conceptual model in which we proposed that clone size potential and sensitivity to gm-CSA are functional properties of granulocyte-macrophage progenitor cells , properties that gradually change as the cells differentiate down the granulocyte-monocyte pathway .
	manualset3
175758	9	410837	13	NULL	NULL	0	NULL	properties	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The major objective of this model was to test an earlier conceptual model in which we proposed that clone size potential and sensitivity to gm-CSA are functional properties of granulocyte-macrophage progenitor cells , properties that gradually change as the cells differentiate down the granulocyte-monocyte pathway .
	manualset3
175759	10	410837	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The major objective of this model was to test an earlier conceptual model in which we proposed that clone size potential and sensitivity to gm-CSA are functional properties of granulocyte-macrophage progenitor cells , properties that gradually change as the cells differentiate down the granulocyte-monocyte pathway .
	manualset3
175760	11	410837	13	NULL	NULL	0	NULL	granulocyte-monocyte pathway	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The major objective of this model was to test an earlier conceptual model in which we proposed that clone size potential and sensitivity to gm-CSA are functional properties of granulocyte-macrophage progenitor cells , properties that gradually change as the cells differentiate down the granulocyte-monocyte pathway .
	manualset3
175908	1	410838	13	NULL	NULL	0	NULL	lung diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The major underlying lung diseases associated with SSP were emphysema ( 22 patients ) and tuberculosis ( 21 patients ) .
	manualset3
175909	2	410838	13	NULL	NULL	0	NULL	SSP 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The major underlying lung diseases associated with SSP were emphysema ( 22 patients ) and tuberculosis ( 21 patients ) .
	manualset3
175910	3	410838	13	NULL	NULL	0	NULL	emphysema	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The major underlying lung diseases associated with SSP were emphysema ( 22 patients ) and tuberculosis ( 21 patients ) .
	manualset3
175911	4	410838	13	NULL	NULL	0	NULL	22 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The major underlying lung diseases associated with SSP were emphysema ( 22 patients ) and tuberculosis ( 21 patients ) .
	manualset3
175912	5	410838	13	NULL	NULL	0	NULL	tuberculosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The major underlying lung diseases associated with SSP were emphysema ( 22 patients ) and tuberculosis ( 21 patients ) .
	manualset3
175913	6	410838	13	NULL	NULL	0	NULL	21 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The major underlying lung diseases associated with SSP were emphysema ( 22 patients ) and tuberculosis ( 21 patients ) .
	manualset3
175914	1	410839	13	NULL	NULL	0	NULL	majority	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of ABC domains energize the transport of compounds across the membranes .
	manualset3
175915	2	410839	13	NULL	NULL	0	NULL	ABC domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of ABC domains energize the transport of compounds across the membranes .
	manualset3
175916	3	410839	13	NULL	NULL	0	NULL	transport 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of ABC domains energize the transport of compounds across the membranes .
	manualset3
175917	4	410839	13	NULL	NULL	0	NULL	compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of ABC domains energize the transport of compounds across the membranes .
	manualset3
175918	5	410839	13	NULL	NULL	0	NULL	membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of ABC domains energize the transport of compounds across the membranes .
	manualset3
175919	1	410840	13	NULL	NULL	0	NULL	majority 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of IC neurons ( 66 % ) displayed an increase in current-evoked action potentials ( Positive Gain ) .
	manualset3
175920	2	410840	13	NULL	NULL	0	NULL	IC neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of IC neurons ( 66 % ) displayed an increase in current-evoked action potentials ( Positive Gain ) .
	manualset3
175921	3	410840	13	NULL	NULL	0	NULL	66 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of IC neurons ( 66 % ) displayed an increase in current-evoked action potentials ( Positive Gain ) .
	manualset3
175922	4	410840	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of IC neurons ( 66 % ) displayed an increase in current-evoked action potentials ( Positive Gain ) .
	manualset3
175923	5	410840	13	NULL	NULL	0	NULL	action potentials	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of IC neurons ( 66 % ) displayed an increase in current-evoked action potentials ( Positive Gain ) .
	manualset3
175924	6	410840	13	NULL	NULL	0	NULL	Positive Gain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of IC neurons ( 66 % ) displayed an increase in current-evoked action potentials ( Positive Gain ) .
	manualset3
175925	1	410841	13	NULL	NULL	0	NULL	majority	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of patients showed symptoms in their early fifties , and men were more commonly affected than women ( ratio of 1.3 : 1 ) .
	manualset3
175926	2	410841	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of patients showed symptoms in their early fifties , and men were more commonly affected than women ( ratio of 1.3 : 1 ) .
	manualset3
175927	3	410841	13	NULL	NULL	0	NULL	symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of patients showed symptoms in their early fifties , and men were more commonly affected than women ( ratio of 1.3 : 1 ) .
	manualset3
175928	4	410841	13	NULL	NULL	0	NULL	 fifties	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of patients showed symptoms in their early fifties , and men were more commonly affected than women ( ratio of 1.3 : 1 ) .
	manualset3
175929	5	410841	13	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of patients showed symptoms in their early fifties , and men were more commonly affected than women ( ratio of 1.3 : 1 ) .
	manualset3
175930	6	410841	13	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of patients showed symptoms in their early fifties , and men were more commonly affected than women ( ratio of 1.3 : 1 ) .
	manualset3
175931	7	410841	13	NULL	NULL	0	NULL	ratio of 1.3 : 1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of patients showed symptoms in their early fifties , and men were more commonly affected than women ( ratio of 1.3 : 1 ) .
	manualset3
175932	1	410842	13	NULL	NULL	0	NULL	majority	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of smoking-cessation programs available to the public uses an effective group format , but it remains underused .
	manualset3
175933	2	410842	13	NULL	NULL	0	NULL	 smoking-cessation programs 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of smoking-cessation programs available to the public uses an effective group format , but it remains underused .
	manualset3
175934	3	410842	13	NULL	NULL	0	NULL	public	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of smoking-cessation programs available to the public uses an effective group format , but it remains underused .
	manualset3
175935	4	410842	13	NULL	NULL	0	NULL	effective group format	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of smoking-cessation programs available to the public uses an effective group format , but it remains underused .
	manualset3
175936	1	410843	13	NULL	NULL	0	NULL	majority 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the ANAE activity in lymphocytes was found to be membrane bound .
	manualset3
175937	2	410843	13	NULL	NULL	0	NULL	ANAE activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the ANAE activity in lymphocytes was found to be membrane bound .
	manualset3
175938	3	410843	13	NULL	NULL	0	NULL	lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the ANAE activity in lymphocytes was found to be membrane bound .
	manualset3
175939	4	410843	13	NULL	NULL	0	NULL	membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the ANAE activity in lymphocytes was found to be membrane bound .
	manualset3
175940	1	410844	13	NULL	NULL	0	NULL	majority 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the Golgi tendon organs , pressure receptors , and the elementary dynamic and static receptors of the muscle spindles did not produce spontaneous discharges .
	manualset3
175941	2	410844	13	NULL	NULL	0	NULL	Golgi tendon organs 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the Golgi tendon organs , pressure receptors , and the elementary dynamic and static receptors of the muscle spindles did not produce spontaneous discharges .
	manualset3
175942	3	410844	13	NULL	NULL	0	NULL	pressure receptors	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the Golgi tendon organs , pressure receptors , and the elementary dynamic and static receptors of the muscle spindles did not produce spontaneous discharges .
	manualset3
175943	4	410844	13	NULL	NULL	0	NULL	 dynamic receptors	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the Golgi tendon organs , pressure receptors , and the elementary dynamic and static receptors of the muscle spindles did not produce spontaneous discharges .
	manualset3
175944	5	410844	13	NULL	NULL	0	NULL	static receptors	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the Golgi tendon organs , pressure receptors , and the elementary dynamic and static receptors of the muscle spindles did not produce spontaneous discharges .
	manualset3
175945	6	410844	13	NULL	NULL	0	NULL	muscle spindles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the Golgi tendon organs , pressure receptors , and the elementary dynamic and static receptors of the muscle spindles did not produce spontaneous discharges .
	manualset3
175946	7	410844	13	NULL	NULL	0	NULL	 spontaneous discharges	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the Golgi tendon organs , pressure receptors , and the elementary dynamic and static receptors of the muscle spindles did not produce spontaneous discharges .
	manualset3
175947	1	410845	13	NULL	NULL	0	NULL	total	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of four oligonucleotides were synthesised for this study , the dimers Tp ( Et ) T and pTp ( Et ) T and the decamer d-TpTpTp ( Et ) TpCpTpApTpTpT together with its unmodified analog .
	manualset3
175948	2	410845	13	NULL	NULL	0	NULL	four	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of four oligonucleotides were synthesised for this study , the dimers Tp ( Et ) T and pTp ( Et ) T and the decamer d-TpTpTp ( Et ) TpCpTpApTpTpT together with its unmodified analog .
	manualset3
175949	3	410845	13	NULL	NULL	0	NULL	oligonucleotides	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of four oligonucleotides were synthesised for this study , the dimers Tp ( Et ) T and pTp ( Et ) T and the decamer d-TpTpTp ( Et ) TpCpTpApTpTpT together with its unmodified analog .
	manualset3
175950	4	410845	13	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of four oligonucleotides were synthesised for this study , the dimers Tp ( Et ) T and pTp ( Et ) T and the decamer d-TpTpTp ( Et ) TpCpTpApTpTpT together with its unmodified analog .
	manualset3
175951	5	410845	13	NULL	NULL	0	NULL	dimers Tp ( Et ) T and pTp ( Et ) T	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of four oligonucleotides were synthesised for this study , the dimers Tp ( Et ) T and pTp ( Et ) T and the decamer d-TpTpTp ( Et ) TpCpTpApTpTpT together with its unmodified analog .
	manualset3
175952	6	410845	13	NULL	NULL	0	NULL	decamer d-TpTpTp ( Et ) TpCpTpApTpTpT	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of four oligonucleotides were synthesised for this study , the dimers Tp ( Et ) T and pTp ( Et ) T and the decamer d-TpTpTp ( Et ) TpCpTpApTpTpT together with its unmodified analog .
	manualset3
175953	7	410845	13	NULL	NULL	0	NULL	analog 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of four oligonucleotides were synthesised for this study , the dimers Tp ( Et ) T and pTp ( Et ) T and the decamer d-TpTpTp ( Et ) TpCpTpApTpTpT together with its unmodified analog .
	manualset3
175954	1	410846	13	NULL	NULL	0	NULL	majority 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the HPeV strains ( n = 15 ) could be identified as HPeV1 , and the remaining 2 strains could be typed as HPeV3 .
	manualset3
175955	2	410846	13	NULL	NULL	0	NULL	HPeV strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the HPeV strains ( n = 15 ) could be identified as HPeV1 , and the remaining 2 strains could be typed as HPeV3 .
	manualset3
175956	3	410846	13	NULL	NULL	0	NULL	n = 15	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the HPeV strains ( n = 15 ) could be identified as HPeV1 , and the remaining 2 strains could be typed as HPeV3 .
	manualset3
175957	4	410846	13	NULL	NULL	0	NULL	HPeV1	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the HPeV strains ( n = 15 ) could be identified as HPeV1 , and the remaining 2 strains could be typed as HPeV3 .
	manualset3
175958	5	410846	13	NULL	NULL	0	NULL	2 strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the HPeV strains ( n = 15 ) could be identified as HPeV1 , and the remaining 2 strains could be typed as HPeV3 .
	manualset3
175959	6	410846	13	NULL	NULL	0	NULL	HPeV3 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the HPeV strains ( n = 15 ) could be identified as HPeV1 , and the remaining 2 strains could be typed as HPeV3 .
	manualset3
175960	1	410847	13	NULL	NULL	0	NULL	 majority	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the airborne bacteria belonged to the genera Bacillus , Micrococcus , and Staphylococcus , but a total of 37 different genera were identified in the air .
	manualset3
175961	2	410847	13	NULL	NULL	0	NULL	 airborne bacteria 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the airborne bacteria belonged to the genera Bacillus , Micrococcus , and Staphylococcus , but a total of 37 different genera were identified in the air .
	manualset3
175962	3	410847	13	NULL	NULL	0	NULL	genera Bacillus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the airborne bacteria belonged to the genera Bacillus , Micrococcus , and Staphylococcus , but a total of 37 different genera were identified in the air .
	manualset3
175963	4	410847	13	NULL	NULL	0	NULL	Micrococcus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the airborne bacteria belonged to the genera Bacillus , Micrococcus , and Staphylococcus , but a total of 37 different genera were identified in the air .
	manualset3
175964	5	410847	13	NULL	NULL	0	NULL	Staphylococcus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the airborne bacteria belonged to the genera Bacillus , Micrococcus , and Staphylococcus , but a total of 37 different genera were identified in the air .
	manualset3
175965	6	410847	13	NULL	NULL	0	NULL	total	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the airborne bacteria belonged to the genera Bacillus , Micrococcus , and Staphylococcus , but a total of 37 different genera were identified in the air .
	manualset3
175966	7	410847	13	NULL	NULL	0	NULL	37 different genera 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the airborne bacteria belonged to the genera Bacillus , Micrococcus , and Staphylococcus , but a total of 37 different genera were identified in the air .
	manualset3
175967	8	410847	13	NULL	NULL	0	NULL	 air	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the airborne bacteria belonged to the genera Bacillus , Micrococcus , and Staphylococcus , but a total of 37 different genera were identified in the air .
	manualset3
175968	1	410848	13	NULL	NULL	0	NULL	majority	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the cells were hyperdistended with mucin , resembling the goblet cells .
	manualset3
175991	2	410848	13	NULL	NULL	0	NULL	 cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the cells were hyperdistended with mucin , resembling the goblet cells .
	manualset3
175994	3	410848	13	NULL	NULL	0	NULL	mucin	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the cells were hyperdistended with mucin , resembling the goblet cells .
	manualset3
175997	4	410848	13	NULL	NULL	0	NULL	goblet cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the cells were hyperdistended with mucin , resembling the goblet cells .
	manualset3
176013	1	410849	13	NULL	NULL	0	NULL	majority	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the sample was white ( 87 % ) , high school or college educated ( 85 % ) , and over half with children ( 56 % ) .
	manualset3
176014	2	410849	13	NULL	NULL	0	NULL	sample 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the sample was white ( 87 % ) , high school or college educated ( 85 % ) , and over half with children ( 56 % ) .
	manualset3
176015	3	410849	13	NULL	NULL	0	NULL	school	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the sample was white ( 87 % ) , high school or college educated ( 85 % ) , and over half with children ( 56 % ) .
	manualset3
176016	4	410849	13	NULL	NULL	0	NULL	 87 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the sample was white ( 87 % ) , high school or college educated ( 85 % ) , and over half with children ( 56 % ) .
	manualset3
176017	5	410849	13	NULL	NULL	0	NULL	college	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the sample was white ( 87 % ) , high school or college educated ( 85 % ) , and over half with children ( 56 % ) .
	manualset3
176018	6	410849	13	NULL	NULL	0	NULL	85 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the sample was white ( 87 % ) , high school or college educated ( 85 % ) , and over half with children ( 56 % ) .
	manualset3
176019	7	410849	13	NULL	NULL	0	NULL	half 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the sample was white ( 87 % ) , high school or college educated ( 85 % ) , and over half with children ( 56 % ) .
	manualset3
176020	8	410849	13	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the sample was white ( 87 % ) , high school or college educated ( 85 % ) , and over half with children ( 56 % ) .
	manualset3
176021	9	410849	13	NULL	NULL	0	NULL	56 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of the sample was white ( 87 % ) , high school or college educated ( 85 % ) , and over half with children ( 56 % ) .
	manualset3
176023	1	410850	13	NULL	NULL	0	NULL	majority	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of tumors in this trial were small , with a median clinical size of 2 cm and a median pathological size of 1.5 cm .
	manualset3
176024	2	410850	13	NULL	NULL	0	NULL	tumors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of tumors in this trial were small , with a median clinical size of 2 cm and a median pathological size of 1.5 cm .
	manualset3
176025	3	410850	13	NULL	NULL	0	NULL	trial	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of tumors in this trial were small , with a median clinical size of 2 cm and a median pathological size of 1.5 cm .
	manualset3
176026	4	410850	13	NULL	NULL	0	NULL	median clinical size 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of tumors in this trial were small , with a median clinical size of 2 cm and a median pathological size of 1.5 cm .
	manualset3
176027	5	410850	13	NULL	NULL	0	NULL	2 cm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of tumors in this trial were small , with a median clinical size of 2 cm and a median pathological size of 1.5 cm .
	manualset3
176028	6	410850	13	NULL	NULL	0	NULL	median pathological size 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of tumors in this trial were small , with a median clinical size of 2 cm and a median pathological size of 1.5 cm .
	manualset3
176029	7	410850	13	NULL	NULL	0	NULL	1.5 cm 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of tumors in this trial were small , with a median clinical size of 2 cm and a median pathological size of 1.5 cm .
	manualset3
176030	1	410851	13	NULL	NULL	0	NULL	toxicogenomic approach	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A toxicogenomic approach to drug-induced phospholipidosis : analysis of its induction mechanism and establishment of a novel in vitro screening system .
	manualset3
176040	2	410851	13	NULL	NULL	0	NULL	drug-induced phospholipidosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A toxicogenomic approach to drug-induced phospholipidosis : analysis of its induction mechanism and establishment of a novel in vitro screening system .
	manualset3
176041	3	410851	13	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A toxicogenomic approach to drug-induced phospholipidosis : analysis of its induction mechanism and establishment of a novel in vitro screening system .
	manualset3
176042	4	410851	13	NULL	NULL	0	NULL	induction mechanism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A toxicogenomic approach to drug-induced phospholipidosis : analysis of its induction mechanism and establishment of a novel in vitro screening system .
	manualset3
176043	5	410851	13	NULL	NULL	0	NULL	establishment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A toxicogenomic approach to drug-induced phospholipidosis : analysis of its induction mechanism and establishment of a novel in vitro screening system .
	manualset3
176044	6	410851	13	NULL	NULL	0	NULL	novel in vitro screening system 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A toxicogenomic approach to drug-induced phospholipidosis : analysis of its induction mechanism and establishment of a novel in vitro screening system .
	manualset3
176045	1	410852	13	NULL	NULL	0	NULL	majority	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of up-regulated genes were involved in metabolism , signal transduction , signalling , transport , and stress response .
	manualset3
176046	2	410852	13	NULL	NULL	0	NULL	up-regulated genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of up-regulated genes were involved in metabolism , signal transduction , signalling , transport , and stress response .
	manualset3
176047	3	410852	13	NULL	NULL	0	NULL	metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of up-regulated genes were involved in metabolism , signal transduction , signalling , transport , and stress response .
	manualset3
176048	4	410852	13	NULL	NULL	0	NULL	signal transduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of up-regulated genes were involved in metabolism , signal transduction , signalling , transport , and stress response .
	manualset3
176049	5	410852	13	NULL	NULL	0	NULL	signalling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of up-regulated genes were involved in metabolism , signal transduction , signalling , transport , and stress response .
	manualset3
176058	6	410852	13	NULL	NULL	0	NULL	transport	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of up-regulated genes were involved in metabolism , signal transduction , signalling , transport , and stress response .
	manualset3
176059	7	410852	13	NULL	NULL	0	NULL	stress response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of up-regulated genes were involved in metabolism , signal transduction , signalling , transport , and stress response .
	manualset3
176060	1	410853	13	NULL	NULL	0	NULL	 majority 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority was found in numerous large phagosomes of macrophages located in the perivascular spaces of the vascular beds and in ependymal cells ( tanycytes ) in the parenchyma .
	manualset3
176061	2	410853	13	NULL	NULL	0	NULL	large phagosomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority was found in numerous large phagosomes of macrophages located in the perivascular spaces of the vascular beds and in ependymal cells ( tanycytes ) in the parenchyma .
	manualset3
176062	3	410853	13	NULL	NULL	0	NULL	macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority was found in numerous large phagosomes of macrophages located in the perivascular spaces of the vascular beds and in ependymal cells ( tanycytes ) in the parenchyma .
	manualset3
176063	4	410853	13	NULL	NULL	0	NULL	 perivascular spaces	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority was found in numerous large phagosomes of macrophages located in the perivascular spaces of the vascular beds and in ependymal cells ( tanycytes ) in the parenchyma .
	manualset3
176064	5	410853	13	NULL	NULL	0	NULL	vascular beds	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority was found in numerous large phagosomes of macrophages located in the perivascular spaces of the vascular beds and in ependymal cells ( tanycytes ) in the parenchyma .
	manualset3
176065	6	410853	13	NULL	NULL	0	NULL	ependymal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority was found in numerous large phagosomes of macrophages located in the perivascular spaces of the vascular beds and in ependymal cells ( tanycytes ) in the parenchyma .
	manualset3
176066	7	410853	13	NULL	NULL	0	NULL	tanycytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority was found in numerous large phagosomes of macrophages located in the perivascular spaces of the vascular beds and in ependymal cells ( tanycytes ) in the parenchyma .
	manualset3
176067	8	410853	13	NULL	NULL	0	NULL	parenchyma	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority was found in numerous large phagosomes of macrophages located in the perivascular spaces of the vascular beds and in ependymal cells ( tanycytes ) in the parenchyma .
	manualset3
176068	1	410854	13	NULL	NULL	NULL	NULL	male bipolar patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The male bipolar patients had significantly larger ventricles , but the depressive patients did not .
	manualset3
176069	2	410854	13	NULL	NULL	0	NULL	ventricles 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The male bipolar patients had significantly larger ventricles , but the depressive patients did not .
	manualset3
176070	3	410854	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The male bipolar patients had significantly larger ventricles , but the depressive patients did not .
	manualset3
176071	1	410855	13	NULL	NULL	0	NULL	male : female seroprevalence ratio	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The male : female seroprevalence ratio was 2 : 1 and the age-group 0-20 years was the most affected .
	manualset3
176072	2	410855	13	NULL	NULL	0	NULL	 2 : 1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The male : female seroprevalence ratio was 2 : 1 and the age-group 0-20 years was the most affected .
	manualset3
176073	3	410855	13	NULL	NULL	0	NULL	age-group 0-20 years	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The male : female seroprevalence ratio was 2 : 1 and the age-group 0-20 years was the most affected .
	manualset3
176074	1	410856	13	NULL	NULL	0	NULL	malignant cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The malignant cells can thereby avoid initiation of potentially dangerous Mvarphi functions and create favorable conditions for tumor progression .
	manualset3
176075	2	410856	13	NULL	NULL	0	NULL	initiation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The malignant cells can thereby avoid initiation of potentially dangerous Mvarphi functions and create favorable conditions for tumor progression .
	manualset3
176076	3	410856	13	NULL	NULL	0	NULL	dangerous Mvarphi functions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The malignant cells can thereby avoid initiation of potentially dangerous Mvarphi functions and create favorable conditions for tumor progression .
	manualset3
176077	4	410856	13	NULL	NULL	0	NULL	conditions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The malignant cells can thereby avoid initiation of potentially dangerous Mvarphi functions and create favorable conditions for tumor progression .
	manualset3
176078	5	410856	13	NULL	NULL	0	NULL	 tumor progression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The malignant cells can thereby avoid initiation of potentially dangerous Mvarphi functions and create favorable conditions for tumor progression .
	manualset3
176084	1	410857	13	NULL	NULL	0	NULL	mammillary complex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The mammillary complex as well as the posterior hypothalamic area represented the most heavily labeled structures in the posterior hypothalamus .
	manualset3
176086	2	410857	13	NULL	NULL	0	NULL	posterior hypothalamic area 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The mammillary complex as well as the posterior hypothalamic area represented the most heavily labeled structures in the posterior hypothalamus .
	manualset3
176087	3	410857	13	NULL	NULL	0	NULL	structures	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The mammillary complex as well as the posterior hypothalamic area represented the most heavily labeled structures in the posterior hypothalamus .
	manualset3
176089	4	410857	13	NULL	NULL	0	NULL	posterior hypothalamus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The mammillary complex as well as the posterior hypothalamic area represented the most heavily labeled structures in the posterior hypothalamus .
	manualset3
176090	1	410858	13	NULL	NULL	0	NULL	toxicologic review 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A toxicologic and dermatologic review of 3-methyl-1-pentanol when used as a fragrance ingredient is presented .
	manualset3
176091	2	410858	13	NULL	NULL	0	NULL	dermatologic review	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A toxicologic and dermatologic review of 3-methyl-1-pentanol when used as a fragrance ingredient is presented .
	manualset3
176092	3	410858	13	NULL	NULL	0	NULL	3-methyl-1-pentanol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A toxicologic and dermatologic review of 3-methyl-1-pentanol when used as a fragrance ingredient is presented .
	manualset3
176093	4	410858	13	NULL	NULL	0	NULL	fragrance ingredient	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A toxicologic and dermatologic review of 3-methyl-1-pentanol when used as a fragrance ingredient is presented .
	manualset3
176094	1	410859	13	NULL	NULL	0	NULL	management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The management of childhood enuresis .
	manualset3
176095	2	410859	13	NULL	NULL	0	NULL	childhood enuresis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The management of childhood enuresis .
	manualset3
176096	1	410860	13	NULL	NULL	0	NULL	mannitol response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The mannitol response is modified by drugs used to prevent EIA , implying that similar mediators are involved .
	manualset3
176097	2	410860	13	NULL	NULL	0	NULL	drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The mannitol response is modified by drugs used to prevent EIA , implying that similar mediators are involved .
	manualset3
176098	3	410860	13	NULL	NULL	0	NULL	EIA	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The mannitol response is modified by drugs used to prevent EIA , implying that similar mediators are involved .
	manualset3
176099	4	410860	13	NULL	NULL	0	NULL	mediator	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The mannitol response is modified by drugs used to prevent EIA , implying that similar mediators are involved .
	manualset3
176101	1	410861	13	NULL	NULL	0	NULL	manubrium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The manubrium was widened using an iliac crest bone graft , stabilised using internal fixation plates and reconstructed with a pectoral muscle flap .
	manualset3
176102	2	410861	13	NULL	NULL	0	NULL	iliac crest bone graft	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The manubrium was widened using an iliac crest bone graft , stabilised using internal fixation plates and reconstructed with a pectoral muscle flap .
	manualset3
176103	3	410861	13	NULL	NULL	0	NULL	internal fixation plates	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The manubrium was widened using an iliac crest bone graft , stabilised using internal fixation plates and reconstructed with a pectoral muscle flap .
	manualset3
176104	4	410861	13	NULL	NULL	0	NULL	pectoral muscle flap	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The manubrium was widened using an iliac crest bone graft , stabilised using internal fixation plates and reconstructed with a pectoral muscle flap .
	manualset3
176105	1	410862	13	NULL	NULL	0	NULL	factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The many factors that control chromatin biology play key roles in essential nuclear functions like transcription , DNA damage response and repair , recombination , and replication and are critical for proper cell-cycle progression , stem cell renewal , differentiation , and development .
	manualset3
176106	2	410862	13	NULL	NULL	NULL	NULL	 chromatin biology	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The many factors that control chromatin biology play key roles in essential nuclear functions like transcription , DNA damage response and repair , recombination , and replication and are critical for proper cell-cycle progression , stem cell renewal , differentiation , and development .
	manualset3
176107	3	410862	13	NULL	NULL	0	NULL	play 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The many factors that control chromatin biology play key roles in essential nuclear functions like transcription , DNA damage response and repair , recombination , and replication and are critical for proper cell-cycle progression , stem cell renewal , differentiation , and development .
	manualset3
176108	4	410862	13	NULL	NULL	0	NULL	 key roles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The many factors that control chromatin biology play key roles in essential nuclear functions like transcription , DNA damage response and repair , recombination , and replication and are critical for proper cell-cycle progression , stem cell renewal , differentiation , and development .
	manualset3
176109	5	410862	13	NULL	NULL	0	NULL	nuclear functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The many factors that control chromatin biology play key roles in essential nuclear functions like transcription , DNA damage response and repair , recombination , and replication and are critical for proper cell-cycle progression , stem cell renewal , differentiation , and development .
	manualset3
176110	6	410862	13	NULL	NULL	NULL	NULL	transcription	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The many factors that control chromatin biology play key roles in essential nuclear functions like transcription , DNA damage response and repair , recombination , and replication and are critical for proper cell-cycle progression , stem cell renewal , differentiation , and development .
	manualset3
176111	7	410862	13	NULL	NULL	0	NULL	DNA damage response 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The many factors that control chromatin biology play key roles in essential nuclear functions like transcription , DNA damage response and repair , recombination , and replication and are critical for proper cell-cycle progression , stem cell renewal , differentiation , and development .
	manualset3
176112	8	410862	13	NULL	NULL	0	NULL	repair	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The many factors that control chromatin biology play key roles in essential nuclear functions like transcription , DNA damage response and repair , recombination , and replication and are critical for proper cell-cycle progression , stem cell renewal , differentiation , and development .
	manualset3
176113	9	410862	13	NULL	NULL	NULL	NULL	recombination	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The many factors that control chromatin biology play key roles in essential nuclear functions like transcription , DNA damage response and repair , recombination , and replication and are critical for proper cell-cycle progression , stem cell renewal , differentiation , and development .
	manualset3
176114	10	410862	13	NULL	NULL	NULL	NULL	replication 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The many factors that control chromatin biology play key roles in essential nuclear functions like transcription , DNA damage response and repair , recombination , and replication and are critical for proper cell-cycle progression , stem cell renewal , differentiation , and development .
	manualset3
176115	11	410862	13	NULL	NULL	0	NULL	cell-cycle progression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The many factors that control chromatin biology play key roles in essential nuclear functions like transcription , DNA damage response and repair , recombination , and replication and are critical for proper cell-cycle progression , stem cell renewal , differentiation , and development .
	manualset3
176116	12	410862	13	NULL	NULL	0	NULL	stem cell renewal	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The many factors that control chromatin biology play key roles in essential nuclear functions like transcription , DNA damage response and repair , recombination , and replication and are critical for proper cell-cycle progression , stem cell renewal , differentiation , and development .
	manualset3
176117	13	410862	13	NULL	NULL	0	NULL	differentiation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The many factors that control chromatin biology play key roles in essential nuclear functions like transcription , DNA damage response and repair , recombination , and replication and are critical for proper cell-cycle progression , stem cell renewal , differentiation , and development .
	manualset3
176118	14	410862	13	NULL	NULL	0	NULL	development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The many factors that control chromatin biology play key roles in essential nuclear functions like transcription , DNA damage response and repair , recombination , and replication and are critical for proper cell-cycle progression , stem cell renewal , differentiation , and development .
	manualset3
176119	1	410863	13	NULL	NULL	0	NULL	goby Pomatoschistus marmoratus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The marbled goby Pomatoschistus marmoratus , a species inhabiting coastal Mediterranean lagoons , has been studied by measuring its mitochondrial DNA variation .
	manualset3
176120	2	410863	13	NULL	NULL	0	NULL	 species 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The marbled goby Pomatoschistus marmoratus , a species inhabiting coastal Mediterranean lagoons , has been studied by measuring its mitochondrial DNA variation .
	manualset3
176121	3	410863	13	NULL	NULL	0	NULL	coastal Mediterranean lagoons	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The marbled goby Pomatoschistus marmoratus , a species inhabiting coastal Mediterranean lagoons , has been studied by measuring its mitochondrial DNA variation .
	manualset3
176122	4	410863	13	NULL	NULL	0	NULL	mitochondrial DNA variation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The marbled goby Pomatoschistus marmoratus , a species inhabiting coastal Mediterranean lagoons , has been studied by measuring its mitochondrial DNA variation .
	manualset3
176123	1	410864	13	NULL	NULL	0	NULL	marine sponge Dysidea avara	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The marine sponge Dysidea avara contained avarol ( 1 ) and avarone ( 2 ) .
	manualset3
176124	2	410864	13	NULL	NULL	0	NULL	avarol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The marine sponge Dysidea avara contained avarol ( 1 ) and avarone ( 2 ) .
	manualset3
176125	3	410864	13	NULL	NULL	0	NULL	avarone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The marine sponge Dysidea avara contained avarol ( 1 ) and avarone ( 2 ) .
	manualset3
176126	1	410865	13	NULL	NULL	0	NULL	markers	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The markers were mapped in a Swedish reference family for gene mapping , comprising eight half-sib families from Standardbred and Icelandic horse sires .
	manualset3
176127	2	410865	13	NULL	NULL	NULL	NULL	 Swedish reference family 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The markers were mapped in a Swedish reference family for gene mapping , comprising eight half-sib families from Standardbred and Icelandic horse sires .
	manualset3
176128	3	410865	13	NULL	NULL	0	NULL	gene mapping 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The markers were mapped in a Swedish reference family for gene mapping , comprising eight half-sib families from Standardbred and Icelandic horse sires .
	manualset3
176129	4	410865	13	NULL	NULL	NULL	NULL	eight half-sib families 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The markers were mapped in a Swedish reference family for gene mapping , comprising eight half-sib families from Standardbred and Icelandic horse sires .
	manualset3
176130	5	410865	13	NULL	NULL	0	NULL	Standardbred sires	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The markers were mapped in a Swedish reference family for gene mapping , comprising eight half-sib families from Standardbred and Icelandic horse sires .
	manualset3
176131	6	410865	13	NULL	NULL	0	NULL	Icelandic horse sires	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The markers were mapped in a Swedish reference family for gene mapping , comprising eight half-sib families from Standardbred and Icelandic horse sires .
	manualset3
176132	1	410866	13	NULL	NULL	0	NULL	mass spectra	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mass spectra of the humic acid fractions were also markedly different from those of the bulk humic acids previously reported .
	manualset3
176133	2	410866	13	NULL	NULL	0	NULL	humic acid fractions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The mass spectra of the humic acid fractions were also markedly different from those of the bulk humic acids previously reported .
	manualset3
176134	3	410866	13	NULL	NULL	0	NULL	 bulk humic acids 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The mass spectra of the humic acid fractions were also markedly different from those of the bulk humic acids previously reported .
	manualset3
176135	1	410867	13	NULL	NULL	0	NULL	inflammation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The massive inflammation of the cerebrospinal fluid ( CSF ) which occurs in adult mice injected with lymphocytic choriomeningitis virus ( LCMV ) has been analyzed by flow microfluorometry ( FMF ) .
	manualset3
176136	2	410867	13	NULL	NULL	0	NULL	cerebrospinal fluid ( CSF )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The massive inflammation of the cerebrospinal fluid ( CSF ) which occurs in adult mice injected with lymphocytic choriomeningitis virus ( LCMV ) has been analyzed by flow microfluorometry ( FMF ) .
	manualset3
176137	3	410867	13	NULL	NULL	0	NULL	adult mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The massive inflammation of the cerebrospinal fluid ( CSF ) which occurs in adult mice injected with lymphocytic choriomeningitis virus ( LCMV ) has been analyzed by flow microfluorometry ( FMF ) .
	manualset3
176138	4	410867	13	NULL	NULL	0	NULL	lymphocytic choriomeningitis virus ( LCMV ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The massive inflammation of the cerebrospinal fluid ( CSF ) which occurs in adult mice injected with lymphocytic choriomeningitis virus ( LCMV ) has been analyzed by flow microfluorometry ( FMF ) .
	manualset3
176139	5	410867	13	NULL	NULL	0	NULL	flow microfluorometry ( FMF )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The massive inflammation of the cerebrospinal fluid ( CSF ) which occurs in adult mice injected with lymphocytic choriomeningitis virus ( LCMV ) has been analyzed by flow microfluorometry ( FMF ) .
	manualset3
176140	1	410868	13	NULL	NULL	0	NULL	 transactivation assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A transactivation assay showed that BIT1 regulates promoter activity of PsbS in a blue light-dependent manner and that it requires CRY1 for activation of the PsbS promoter .
	manualset3
176141	2	410868	13	NULL	NULL	0	NULL	BIT1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A transactivation assay showed that BIT1 regulates promoter activity of PsbS in a blue light-dependent manner and that it requires CRY1 for activation of the PsbS promoter .
	manualset3
176142	3	410868	13	NULL	NULL	0	NULL	promoter activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A transactivation assay showed that BIT1 regulates promoter activity of PsbS in a blue light-dependent manner and that it requires CRY1 for activation of the PsbS promoter .
	manualset3
176143	4	410868	13	NULL	NULL	0	NULL	PsbS	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A transactivation assay showed that BIT1 regulates promoter activity of PsbS in a blue light-dependent manner and that it requires CRY1 for activation of the PsbS promoter .
	manualset3
176144	5	410868	13	NULL	NULL	0	NULL	blue light-dependent manner 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A transactivation assay showed that BIT1 regulates promoter activity of PsbS in a blue light-dependent manner and that it requires CRY1 for activation of the PsbS promoter .
	manualset3
176145	6	410868	13	NULL	NULL	0	NULL	CRY1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A transactivation assay showed that BIT1 regulates promoter activity of PsbS in a blue light-dependent manner and that it requires CRY1 for activation of the PsbS promoter .
	manualset3
176146	7	410868	13	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A transactivation assay showed that BIT1 regulates promoter activity of PsbS in a blue light-dependent manner and that it requires CRY1 for activation of the PsbS promoter .
	manualset3
176147	8	410868	13	NULL	NULL	0	NULL	PsbS promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A transactivation assay showed that BIT1 regulates promoter activity of PsbS in a blue light-dependent manner and that it requires CRY1 for activation of the PsbS promoter .
	manualset3
176148	1	410869	13	NULL	NULL	0	NULL	mast cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The mast cells : distribution and morphology .
	manualset3
176149	2	410869	13	NULL	NULL	0	NULL	distribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mast cells : distribution and morphology .
	manualset3
176150	3	410869	13	NULL	NULL	0	NULL	morphology	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mast cells : distribution and morphology .
	manualset3
176151	1	410870	13	NULL	NULL	0	NULL	material measurements	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The material measurements diverged logically from the clothing measurements but material methods had a better capability to analyze the differences of material ensembles .
	manualset3
176152	2	410870	13	NULL	NULL	0	NULL	clothing measurements	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The material measurements diverged logically from the clothing measurements but material methods had a better capability to analyze the differences of material ensembles .
	manualset3
176153	3	410870	13	NULL	NULL	0	NULL	material methods	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The material measurements diverged logically from the clothing measurements but material methods had a better capability to analyze the differences of material ensembles .
	manualset3
176154	4	410870	13	NULL	NULL	0	NULL	capability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The material measurements diverged logically from the clothing measurements but material methods had a better capability to analyze the differences of material ensembles .
	manualset3
176155	5	410870	13	NULL	NULL	0	NULL	differences 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The material measurements diverged logically from the clothing measurements but material methods had a better capability to analyze the differences of material ensembles .
	manualset3
176156	6	410870	13	NULL	NULL	0	NULL	material ensembles 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The material measurements diverged logically from the clothing measurements but material methods had a better capability to analyze the differences of material ensembles .
	manualset3
176157	1	410871	13	NULL	NULL	0	NULL	 material strength	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The material strength of the humerus was greater than the tibiotarsus ; this difference in strength was reflected in both the collagen and mineral matrix biochemistry .
	manualset3
176158	2	410871	13	NULL	NULL	0	NULL	humerus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The material strength of the humerus was greater than the tibiotarsus ; this difference in strength was reflected in both the collagen and mineral matrix biochemistry .
	manualset3
176159	3	410871	13	NULL	NULL	0	NULL	tibiotarsus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The material strength of the humerus was greater than the tibiotarsus ; this difference in strength was reflected in both the collagen and mineral matrix biochemistry .
	manualset3
176160	4	410871	13	NULL	NULL	0	NULL	difference 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The material strength of the humerus was greater than the tibiotarsus ; this difference in strength was reflected in both the collagen and mineral matrix biochemistry .
	manualset3
176161	5	410871	13	NULL	NULL	0	NULL	strength 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The material strength of the humerus was greater than the tibiotarsus ; this difference in strength was reflected in both the collagen and mineral matrix biochemistry .
	manualset3
176162	6	410871	13	NULL	NULL	0	NULL	collagen 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The material strength of the humerus was greater than the tibiotarsus ; this difference in strength was reflected in both the collagen and mineral matrix biochemistry .
	manualset3
176163	7	410871	13	NULL	NULL	0	NULL	 mineral matrix biochemistry 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The material strength of the humerus was greater than the tibiotarsus ; this difference in strength was reflected in both the collagen and mineral matrix biochemistry .
	manualset3
176166	1	410872	13	NULL	NULL	0	NULL	mature LAP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mature LAP is preceded by a leader peptide of 77 amino acids , predicted to include an 18-amino-acid signal peptide and an extra sequence of 59 amino acids .
	manualset3
176169	2	410872	13	NULL	NULL	0	NULL	leader peptide of 77 amino acids	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The mature LAP is preceded by a leader peptide of 77 amino acids , predicted to include an 18-amino-acid signal peptide and an extra sequence of 59 amino acids .
	manualset3
176171	3	410872	13	NULL	NULL	0	NULL	18-amino-acid signal peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The mature LAP is preceded by a leader peptide of 77 amino acids , predicted to include an 18-amino-acid signal peptide and an extra sequence of 59 amino acids .
	manualset3
176172	4	410872	13	NULL	NULL	0	NULL	sequence of 59 amino acids 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The mature LAP is preceded by a leader peptide of 77 amino acids , predicted to include an 18-amino-acid signal peptide and an extra sequence of 59 amino acids .
	manualset3
176175	1	410873	13	NULL	NULL	0	NULL	mature form	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mature form of the MuIFN-alpha 1 protein was expressed as well as analog forms with amino acid substitutions at positions 33 , 71 , 72 , 123 and 133 .
	manualset3
176177	2	410873	13	NULL	NULL	0	NULL	MuIFN-alpha 1 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mature form of the MuIFN-alpha 1 protein was expressed as well as analog forms with amino acid substitutions at positions 33 , 71 , 72 , 123 and 133 .
	manualset3
176178	3	410873	13	NULL	NULL	0	NULL	analog forms 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The mature form of the MuIFN-alpha 1 protein was expressed as well as analog forms with amino acid substitutions at positions 33 , 71 , 72 , 123 and 133 .
	manualset3
176179	4	410873	13	NULL	NULL	0	NULL	amino acid substitutions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mature form of the MuIFN-alpha 1 protein was expressed as well as analog forms with amino acid substitutions at positions 33 , 71 , 72 , 123 and 133 .
	manualset3
176182	5	410873	13	NULL	NULL	NULL	NULL	positions 33	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The mature form of the MuIFN-alpha 1 protein was expressed as well as analog forms with amino acid substitutions at positions 33 , 71 , 72 , 123 and 133 .
	manualset3
176187	6	410873	13	NULL	NULL	0	NULL	positions 71	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mature form of the MuIFN-alpha 1 protein was expressed as well as analog forms with amino acid substitutions at positions 33 , 71 , 72 , 123 and 133 .
	manualset3
176188	7	410873	13	NULL	NULL	0	NULL	positions 72	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mature form of the MuIFN-alpha 1 protein was expressed as well as analog forms with amino acid substitutions at positions 33 , 71 , 72 , 123 and 133 .
	manualset3
176189	8	410873	13	NULL	NULL	0	NULL	positions 123	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mature form of the MuIFN-alpha 1 protein was expressed as well as analog forms with amino acid substitutions at positions 33 , 71 , 72 , 123 and 133 .
	manualset3
176191	9	410873	13	NULL	NULL	0	NULL	positions 133	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mature form of the MuIFN-alpha 1 protein was expressed as well as analog forms with amino acid substitutions at positions 33 , 71 , 72 , 123 and 133 .
	manualset3
176197	1	410874	13	NULL	NULL	0	NULL	mature wild-type VSV G protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mature wild-type VSV G protein is a noncovalently associated trimer .
	manualset3
176199	2	410874	13	NULL	NULL	0	NULL	trimer 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mature wild-type VSV G protein is a noncovalently associated trimer .
	manualset3
176205	1	410875	13	NULL	NULL	0	NULL	mauJ product 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mauJ product is the only polypeptide encoded by the mau gene cluster which is predicted to be cytoplasmic .
	manualset3
176207	2	410875	13	NULL	NULL	0	NULL	polypeptide 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The mauJ product is the only polypeptide encoded by the mau gene cluster which is predicted to be cytoplasmic .
	manualset3
176210	3	410875	13	NULL	NULL	0	NULL	mau gene cluster	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The mauJ product is the only polypeptide encoded by the mau gene cluster which is predicted to be cytoplasmic .
	manualset3
176214	1	410876	13	NULL	NULL	0	NULL	maxillary tuberosity region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The maxillary tuberosity region is becoming increasingly involved in preprosthetic surgery as part of a comprehensive implant treatment planning .
	manualset3
176215	2	410876	13	NULL	NULL	0	NULL	preprosthetic surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The maxillary tuberosity region is becoming increasingly involved in preprosthetic surgery as part of a comprehensive implant treatment planning .
	manualset3
176216	3	410876	13	NULL	NULL	0	NULL	part 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The maxillary tuberosity region is becoming increasingly involved in preprosthetic surgery as part of a comprehensive implant treatment planning .
	manualset3
176217	4	410876	13	NULL	NULL	0	NULL	comprehensive implant treatment planning	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The maxillary tuberosity region is becoming increasingly involved in preprosthetic surgery as part of a comprehensive implant treatment planning .
	manualset3
176224	1	410877	13	NULL	NULL	0	NULL	maximal physiological responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximal physiological responses to treadmill running ( TMR ) , shallow water running ( SWR ) and deep water running ( DWR ) while wearing a buoyancy vest were compared in 15 trained male runners .
	manualset3
176229	2	410877	13	NULL	NULL	NULL	NULL	treadmill running ( TMR )	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The maximal physiological responses to treadmill running ( TMR ) , shallow water running ( SWR ) and deep water running ( DWR ) while wearing a buoyancy vest were compared in 15 trained male runners .
	manualset3
176231	3	410877	13	NULL	NULL	NULL	NULL	shallow water running ( SWR )	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The maximal physiological responses to treadmill running ( TMR ) , shallow water running ( SWR ) and deep water running ( DWR ) while wearing a buoyancy vest were compared in 15 trained male runners .
	manualset3
176234	4	410877	13	NULL	NULL	NULL	NULL	deep water running ( DWR )	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The maximal physiological responses to treadmill running ( TMR ) , shallow water running ( SWR ) and deep water running ( DWR ) while wearing a buoyancy vest were compared in 15 trained male runners .
	manualset3
176244	5	410877	13	NULL	NULL	0	NULL	buoyancy vest 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximal physiological responses to treadmill running ( TMR ) , shallow water running ( SWR ) and deep water running ( DWR ) while wearing a buoyancy vest were compared in 15 trained male runners .
	manualset3
176246	6	410877	13	NULL	NULL	0	NULL	15 trained male runners	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximal physiological responses to treadmill running ( TMR ) , shallow water running ( SWR ) and deep water running ( DWR ) while wearing a buoyancy vest were compared in 15 trained male runners .
	manualset3
176248	1	410878	13	NULL	NULL	0	NULL	suppression 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A transient but marked suppression in the excitability of the parallel fiber-Purkinje cell circuitry accompanied the spread .
	manualset3
176250	2	410878	13	NULL	NULL	0	NULL	excitability 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A transient but marked suppression in the excitability of the parallel fiber-Purkinje cell circuitry accompanied the spread .
	manualset3
176251	3	410878	13	NULL	NULL	0	NULL	parallel fiber-Purkinje cell circuitry 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A transient but marked suppression in the excitability of the parallel fiber-Purkinje cell circuitry accompanied the spread .
	manualset3
176252	1	410879	13	NULL	NULL	0	NULL	adsorption 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum adsorption of BSA on magnetic particles occurred at the isoelectric point of BSA .
	manualset3
176253	2	410879	13	NULL	NULL	0	NULL	BSA 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum adsorption of BSA on magnetic particles occurred at the isoelectric point of BSA .
	manualset3
176254	3	410879	13	NULL	NULL	0	NULL	magnetic particles 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum adsorption of BSA on magnetic particles occurred at the isoelectric point of BSA .
	manualset3
176255	4	410879	13	NULL	NULL	0	NULL	isoelectric point	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum adsorption of BSA on magnetic particles occurred at the isoelectric point of BSA .
	manualset3
176256	5	410879	13	NULL	NULL	0	NULL	BSA 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum adsorption of BSA on magnetic particles occurred at the isoelectric point of BSA .
	manualset3
176299	1	410880	13	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum increase in late potential duration ( LPD ) was threefold greater than the increase in filtered QRS duration or QTc ( 61 % vs 18 % vs 14 % , respectively ) , suggesting a more pronounced effect on the reentrant pathway than on the remaining myocardium .
	manualset3
176300	2	410880	13	NULL	NULL	0	NULL	late potential duration ( LPD ) 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum increase in late potential duration ( LPD ) was threefold greater than the increase in filtered QRS duration or QTc ( 61 % vs 18 % vs 14 % , respectively ) , suggesting a more pronounced effect on the reentrant pathway than on the remaining myocardium .
	manualset3
176301	3	410880	13	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum increase in late potential duration ( LPD ) was threefold greater than the increase in filtered QRS duration or QTc ( 61 % vs 18 % vs 14 % , respectively ) , suggesting a more pronounced effect on the reentrant pathway than on the remaining myocardium .
	manualset3
176302	4	410880	13	NULL	NULL	0	NULL	QRS duration 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum increase in late potential duration ( LPD ) was threefold greater than the increase in filtered QRS duration or QTc ( 61 % vs 18 % vs 14 % , respectively ) , suggesting a more pronounced effect on the reentrant pathway than on the remaining myocardium .
	manualset3
176303	5	410880	13	NULL	NULL	NULL	NULL	QTc 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The maximum increase in late potential duration ( LPD ) was threefold greater than the increase in filtered QRS duration or QTc ( 61 % vs 18 % vs 14 % , respectively ) , suggesting a more pronounced effect on the reentrant pathway than on the remaining myocardium .
	manualset3
176304	6	410880	13	NULL	NULL	0	NULL	61 % vs 18 % vs 14 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum increase in late potential duration ( LPD ) was threefold greater than the increase in filtered QRS duration or QTc ( 61 % vs 18 % vs 14 % , respectively ) , suggesting a more pronounced effect on the reentrant pathway than on the remaining myocardium .
	manualset3
176305	7	410880	13	NULL	NULL	0	NULL	effect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum increase in late potential duration ( LPD ) was threefold greater than the increase in filtered QRS duration or QTc ( 61 % vs 18 % vs 14 % , respectively ) , suggesting a more pronounced effect on the reentrant pathway than on the remaining myocardium .
	manualset3
176306	8	410880	13	NULL	NULL	0	NULL	reentrant pathway	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum increase in late potential duration ( LPD ) was threefold greater than the increase in filtered QRS duration or QTc ( 61 % vs 18 % vs 14 % , respectively ) , suggesting a more pronounced effect on the reentrant pathway than on the remaining myocardium .
	manualset3
176307	9	410880	13	NULL	NULL	0	NULL	myocardium 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum increase in late potential duration ( LPD ) was threefold greater than the increase in filtered QRS duration or QTc ( 61 % vs 18 % vs 14 % , respectively ) , suggesting a more pronounced effect on the reentrant pathway than on the remaining myocardium .
	manualset3
176308	1	410881	13	NULL	NULL	0	NULL	concentrations 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum inhibitory concentrations of Cys , CysOME , CysOEt and N-AcCys showed a positive relationship to the pKa ( RSH ) values of the thiols and those of CysOEt and Cys decreased with increasing pH. .
	manualset3
176309	2	410881	13	NULL	NULL	0	NULL	Cys 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum inhibitory concentrations of Cys , CysOME , CysOEt and N-AcCys showed a positive relationship to the pKa ( RSH ) values of the thiols and those of CysOEt and Cys decreased with increasing pH. .
	manualset3
176310	3	410881	13	NULL	NULL	NULL	NULL	CysOME 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The maximum inhibitory concentrations of Cys , CysOME , CysOEt and N-AcCys showed a positive relationship to the pKa ( RSH ) values of the thiols and those of CysOEt and Cys decreased with increasing pH. .
	manualset3
176311	4	410881	13	NULL	NULL	0	NULL	CysOEt 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum inhibitory concentrations of Cys , CysOME , CysOEt and N-AcCys showed a positive relationship to the pKa ( RSH ) values of the thiols and those of CysOEt and Cys decreased with increasing pH. .
	manualset3
176312	5	410881	13	NULL	NULL	0	NULL	N-AcCys	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum inhibitory concentrations of Cys , CysOME , CysOEt and N-AcCys showed a positive relationship to the pKa ( RSH ) values of the thiols and those of CysOEt and Cys decreased with increasing pH. .
	manualset3
176313	6	410881	13	NULL	NULL	0	NULL	relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum inhibitory concentrations of Cys , CysOME , CysOEt and N-AcCys showed a positive relationship to the pKa ( RSH ) values of the thiols and those of CysOEt and Cys decreased with increasing pH. .
	manualset3
176314	7	410881	13	NULL	NULL	0	NULL	pKa ( RSH ) values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum inhibitory concentrations of Cys , CysOME , CysOEt and N-AcCys showed a positive relationship to the pKa ( RSH ) values of the thiols and those of CysOEt and Cys decreased with increasing pH. .
	manualset3
176315	8	410881	13	NULL	NULL	0	NULL	thiols 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum inhibitory concentrations of Cys , CysOME , CysOEt and N-AcCys showed a positive relationship to the pKa ( RSH ) values of the thiols and those of CysOEt and Cys decreased with increasing pH. .
	manualset3
176316	9	410881	13	NULL	NULL	0	NULL	CysOEt 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum inhibitory concentrations of Cys , CysOME , CysOEt and N-AcCys showed a positive relationship to the pKa ( RSH ) values of the thiols and those of CysOEt and Cys decreased with increasing pH. .
	manualset3
176317	10	410881	13	NULL	NULL	0	NULL	Cys 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum inhibitory concentrations of Cys , CysOME , CysOEt and N-AcCys showed a positive relationship to the pKa ( RSH ) values of the thiols and those of CysOEt and Cys decreased with increasing pH. .
	manualset3
176318	11	410881	13	NULL	NULL	0	NULL	pH	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum inhibitory concentrations of Cys , CysOME , CysOEt and N-AcCys showed a positive relationship to the pKa ( RSH ) values of the thiols and those of CysOEt and Cys decreased with increasing pH. .
	manualset3
176319	1	410882	13	NULL	NULL	0	NULL	levels 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum levels of ( Ca2 + ) i induced by the three points were ET-1 approximately equal to ET-2 ) ET-3 .
	manualset3
176320	2	410882	13	NULL	NULL	0	NULL	( Ca2 + ) i	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum levels of ( Ca2 + ) i induced by the three points were ET-1 approximately equal to ET-2 ) ET-3 .
	manualset3
176321	3	410882	13	NULL	NULL	0	NULL	three points 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum levels of ( Ca2 + ) i induced by the three points were ET-1 approximately equal to ET-2 ) ET-3 .
	manualset3
176322	4	410882	13	NULL	NULL	0	NULL	ET-1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum levels of ( Ca2 + ) i induced by the three points were ET-1 approximately equal to ET-2 ) ET-3 .
	manualset3
176323	5	410882	13	NULL	NULL	0	NULL	ET-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum levels of ( Ca2 + ) i induced by the three points were ET-1 approximately equal to ET-2 ) ET-3 .
	manualset3
176324	6	410882	13	NULL	NULL	0	NULL	ET-3 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum levels of ( Ca2 + ) i induced by the three points were ET-1 approximately equal to ET-2 ) ET-3 .
	manualset3
176325	1	410883	13	NULL	NULL	0	NULL	motor fiber	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum motor fiber conduction velocity and the distal latency were measured every two weeks in the tail nerves of the treated animals and controls .
	manualset3
176326	2	410883	13	NULL	NULL	0	NULL	conduction velocity 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum motor fiber conduction velocity and the distal latency were measured every two weeks in the tail nerves of the treated animals and controls .
	manualset3
176327	3	410883	13	NULL	NULL	0	NULL	distal latency	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum motor fiber conduction velocity and the distal latency were measured every two weeks in the tail nerves of the treated animals and controls .
	manualset3
176328	4	410883	13	NULL	NULL	0	NULL	two weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum motor fiber conduction velocity and the distal latency were measured every two weeks in the tail nerves of the treated animals and controls .
	manualset3
176329	5	410883	13	NULL	NULL	0	NULL	tail nerves	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum motor fiber conduction velocity and the distal latency were measured every two weeks in the tail nerves of the treated animals and controls .
	manualset3
176330	6	410883	13	NULL	NULL	0	NULL	animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum motor fiber conduction velocity and the distal latency were measured every two weeks in the tail nerves of the treated animals and controls .
	manualset3
176331	7	410883	13	NULL	NULL	0	NULL	controls 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum motor fiber conduction velocity and the distal latency were measured every two weeks in the tail nerves of the treated animals and controls .
	manualset3
176332	1	410884	13	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum number of ligands that can be bound to HSA is 9 for PFOA and 11 for PFOS .
	manualset3
176333	2	410884	13	NULL	NULL	0	NULL	ligands 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum number of ligands that can be bound to HSA is 9 for PFOA and 11 for PFOS .
	manualset3
176334	3	410884	13	NULL	NULL	0	NULL	HSA 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum number of ligands that can be bound to HSA is 9 for PFOA and 11 for PFOS .
	manualset3
176335	4	410884	13	NULL	NULL	0	NULL	9 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum number of ligands that can be bound to HSA is 9 for PFOA and 11 for PFOS .
	manualset3
176336	5	410884	13	NULL	NULL	0	NULL	PFOA 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum number of ligands that can be bound to HSA is 9 for PFOA and 11 for PFOS .
	manualset3
176337	6	410884	13	NULL	NULL	0	NULL	11 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum number of ligands that can be bound to HSA is 9 for PFOA and 11 for PFOS .
	manualset3
176338	7	410884	13	NULL	NULL	0	NULL	PFOS 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum number of ligands that can be bound to HSA is 9 for PFOA and 11 for PFOS .
	manualset3
176339	1	410885	13	NULL	NULL	0	NULL	maximum reflection loss	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum reflection loss of the BaTiO ( 3 ) nano-torus reached -28.38 dB at 11.36 GHz , compared to that of -12.87 dB at 16.32 GHz of the BaTiO ( 3 ) solid nanoparticles .
	manualset3
176340	2	410885	13	NULL	NULL	0	NULL	BaTiO ( 3 ) nano-torus	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum reflection loss of the BaTiO ( 3 ) nano-torus reached -28.38 dB at 11.36 GHz , compared to that of -12.87 dB at 16.32 GHz of the BaTiO ( 3 ) solid nanoparticles .
	manualset3
176341	3	410885	13	NULL	NULL	0	NULL	-28.38 dB 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum reflection loss of the BaTiO ( 3 ) nano-torus reached -28.38 dB at 11.36 GHz , compared to that of -12.87 dB at 16.32 GHz of the BaTiO ( 3 ) solid nanoparticles .
	manualset3
176342	4	410885	13	NULL	NULL	0	NULL	11.36 GHz	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum reflection loss of the BaTiO ( 3 ) nano-torus reached -28.38 dB at 11.36 GHz , compared to that of -12.87 dB at 16.32 GHz of the BaTiO ( 3 ) solid nanoparticles .
	manualset3
176343	5	410885	13	NULL	NULL	0	NULL	-12.87 dB 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum reflection loss of the BaTiO ( 3 ) nano-torus reached -28.38 dB at 11.36 GHz , compared to that of -12.87 dB at 16.32 GHz of the BaTiO ( 3 ) solid nanoparticles .
	manualset3
176344	6	410885	13	NULL	NULL	0	NULL	16.32 GHz	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum reflection loss of the BaTiO ( 3 ) nano-torus reached -28.38 dB at 11.36 GHz , compared to that of -12.87 dB at 16.32 GHz of the BaTiO ( 3 ) solid nanoparticles .
	manualset3
176345	7	410885	13	NULL	NULL	0	NULL	BaTiO ( 3 ) solid nanoparticles 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum reflection loss of the BaTiO ( 3 ) nano-torus reached -28.38 dB at 11.36 GHz , compared to that of -12.87 dB at 16.32 GHz of the BaTiO ( 3 ) solid nanoparticles .
	manualset3
176346	1	410886	13	NULL	NULL	0	NULL	maximum scattering coefficients	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum scattering coefficients for normal and adenomatous colon mucosa/submucosa are 890 nm , and the minimum scattering coefficients for both are 780 nm .
	manualset3
176347	2	410886	13	NULL	NULL	0	NULL	adenomatous colon mucosa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum scattering coefficients for normal and adenomatous colon mucosa/submucosa are 890 nm , and the minimum scattering coefficients for both are 780 nm .
	manualset3
176348	3	410886	13	NULL	NULL	0	NULL	adenomatous colon submucosa 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum scattering coefficients for normal and adenomatous colon mucosa/submucosa are 890 nm , and the minimum scattering coefficients for both are 780 nm .
	manualset3
176349	4	410886	13	NULL	NULL	0	NULL	890 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum scattering coefficients for normal and adenomatous colon mucosa/submucosa are 890 nm , and the minimum scattering coefficients for both are 780 nm .
	manualset3
176350	5	410886	13	NULL	NULL	0	NULL	minimum scattering coefficients 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum scattering coefficients for normal and adenomatous colon mucosa/submucosa are 890 nm , and the minimum scattering coefficients for both are 780 nm .
	manualset3
176351	6	410886	13	NULL	NULL	0	NULL	780 nm 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum scattering coefficients for normal and adenomatous colon mucosa/submucosa are 890 nm , and the minimum scattering coefficients for both are 780 nm .
	manualset3
176352	1	410887	13	NULL	NULL	0	NULL	transitory decrease 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A transitory , ipsilateral decrease was also observed in the caudate-putamen and the somato-sensory cortex , likely due to involvement of polysynaptic pathways .
	manualset3
176353	2	410887	13	NULL	NULL	0	NULL	ipsilateral decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A transitory , ipsilateral decrease was also observed in the caudate-putamen and the somato-sensory cortex , likely due to involvement of polysynaptic pathways .
	manualset3
176354	3	410887	13	NULL	NULL	0	NULL	caudate-putamen cortex 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A transitory , ipsilateral decrease was also observed in the caudate-putamen and the somato-sensory cortex , likely due to involvement of polysynaptic pathways .
	manualset3
176355	4	410887	13	NULL	NULL	0	NULL	somato-sensory cortex 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A transitory , ipsilateral decrease was also observed in the caudate-putamen and the somato-sensory cortex , likely due to involvement of polysynaptic pathways .
	manualset3
176356	5	410887	13	NULL	NULL	0	NULL	involvement 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A transitory , ipsilateral decrease was also observed in the caudate-putamen and the somato-sensory cortex , likely due to involvement of polysynaptic pathways .
	manualset3
176357	6	410887	13	NULL	NULL	0	NULL	polysynaptic pathways 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A transitory , ipsilateral decrease was also observed in the caudate-putamen and the somato-sensory cortex , likely due to involvement of polysynaptic pathways .
	manualset3
176403	1	410888	13	NULL	NULL	0	NULL	maximum transport capacity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum transport capacity of acetate through the BBB ( V ( max ) ( t ) = 0.96 + / - 0.18 micromol/g/min ) was nearly twofold higher than the maximum rate of brain acetate utilization ( V ( max ) ( util ) = 0.50 + / - 0.08 micromol/g/min ) .
	manualset3
176404	2	410888	13	NULL	NULL	0	NULL	acetate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum transport capacity of acetate through the BBB ( V ( max ) ( t ) = 0.96 + / - 0.18 micromol/g/min ) was nearly twofold higher than the maximum rate of brain acetate utilization ( V ( max ) ( util ) = 0.50 + / - 0.08 micromol/g/min ) .
	manualset3
176405	3	410888	13	NULL	NULL	0	NULL	BBB	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum transport capacity of acetate through the BBB ( V ( max ) ( t ) = 0.96 + / - 0.18 micromol/g/min ) was nearly twofold higher than the maximum rate of brain acetate utilization ( V ( max ) ( util ) = 0.50 + / - 0.08 micromol/g/min ) .
	manualset3
176406	4	410888	13	NULL	NULL	0	NULL	 V ( max ) ( t ) = 0.96 + / - 0.18 micromol/g/min	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum transport capacity of acetate through the BBB ( V ( max ) ( t ) = 0.96 + / - 0.18 micromol/g/min ) was nearly twofold higher than the maximum rate of brain acetate utilization ( V ( max ) ( util ) = 0.50 + / - 0.08 micromol/g/min ) .
	manualset3
176407	5	410888	13	NULL	NULL	NULL	NULL	rate	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The maximum transport capacity of acetate through the BBB ( V ( max ) ( t ) = 0.96 + / - 0.18 micromol/g/min ) was nearly twofold higher than the maximum rate of brain acetate utilization ( V ( max ) ( util ) = 0.50 + / - 0.08 micromol/g/min ) .
	manualset3
176408	6	410888	13	NULL	NULL	0	NULL	brain acetate utilization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum transport capacity of acetate through the BBB ( V ( max ) ( t ) = 0.96 + / - 0.18 micromol/g/min ) was nearly twofold higher than the maximum rate of brain acetate utilization ( V ( max ) ( util ) = 0.50 + / - 0.08 micromol/g/min ) .
	manualset3
176409	7	410888	13	NULL	NULL	0	NULL	V ( max ) ( util ) = 0.50 + / - 0.08 micromol/g/min	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The maximum transport capacity of acetate through the BBB ( V ( max ) ( t ) = 0.96 + / - 0.18 micromol/g/min ) was nearly twofold higher than the maximum rate of brain acetate utilization ( V ( max ) ( util ) = 0.50 + / - 0.08 micromol/g/min ) .
	manualset3
176410	1	410889	13	NULL	NULL	0	NULL	mean 18-month 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean 18-month follow-up showed two early cardiac deaths and 12 additional myocardial infarctions .
	manualset3
176411	2	410889	13	NULL	NULL	0	NULL	follow-up	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean 18-month follow-up showed two early cardiac deaths and 12 additional myocardial infarctions .
	manualset3
176412	3	410889	13	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean 18-month follow-up showed two early cardiac deaths and 12 additional myocardial infarctions .
	manualset3
176413	4	410889	13	NULL	NULL	0	NULL	cardiac deaths	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean 18-month follow-up showed two early cardiac deaths and 12 additional myocardial infarctions .
	manualset3
176414	5	410889	13	NULL	NULL	0	NULL	12	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean 18-month follow-up showed two early cardiac deaths and 12 additional myocardial infarctions .
	manualset3
176415	6	410889	13	NULL	NULL	0	NULL	myocardial infarctions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean 18-month follow-up showed two early cardiac deaths and 12 additional myocardial infarctions .
	manualset3
176416	1	410890	13	NULL	NULL	0	NULL	mean APACHE II score	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean APACHE II score on admission was 18.8 , the mean Charlson comorbidity index was 2.9 , and 20 ( 95.2 % ) patients had a history of intensive care unit hospitalization .
	manualset3
176417	2	410890	13	NULL	NULL	0	NULL	admission	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean APACHE II score on admission was 18.8 , the mean Charlson comorbidity index was 2.9 , and 20 ( 95.2 % ) patients had a history of intensive care unit hospitalization .
	manualset3
176418	3	410890	13	NULL	NULL	0	NULL	18.8	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean APACHE II score on admission was 18.8 , the mean Charlson comorbidity index was 2.9 , and 20 ( 95.2 % ) patients had a history of intensive care unit hospitalization .
	manualset3
176419	4	410890	13	NULL	NULL	0	NULL	 mean Charlson comorbidity index 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean APACHE II score on admission was 18.8 , the mean Charlson comorbidity index was 2.9 , and 20 ( 95.2 % ) patients had a history of intensive care unit hospitalization .
	manualset3
176420	5	410890	13	NULL	NULL	0	NULL	2.9	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean APACHE II score on admission was 18.8 , the mean Charlson comorbidity index was 2.9 , and 20 ( 95.2 % ) patients had a history of intensive care unit hospitalization .
	manualset3
176421	6	410890	13	NULL	NULL	0	NULL	20 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean APACHE II score on admission was 18.8 , the mean Charlson comorbidity index was 2.9 , and 20 ( 95.2 % ) patients had a history of intensive care unit hospitalization .
	manualset3
176422	7	410890	13	NULL	NULL	0	NULL	95.2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean APACHE II score on admission was 18.8 , the mean Charlson comorbidity index was 2.9 , and 20 ( 95.2 % ) patients had a history of intensive care unit hospitalization .
	manualset3
176423	8	410890	13	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean APACHE II score on admission was 18.8 , the mean Charlson comorbidity index was 2.9 , and 20 ( 95.2 % ) patients had a history of intensive care unit hospitalization .
	manualset3
176424	9	410890	13	NULL	NULL	0	NULL	history 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean APACHE II score on admission was 18.8 , the mean Charlson comorbidity index was 2.9 , and 20 ( 95.2 % ) patients had a history of intensive care unit hospitalization .
	manualset3
176425	10	410890	13	NULL	NULL	0	NULL	intensive care unit	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean APACHE II score on admission was 18.8 , the mean Charlson comorbidity index was 2.9 , and 20 ( 95.2 % ) patients had a history of intensive care unit hospitalization .
	manualset3
176426	11	410890	13	NULL	NULL	0	NULL	hospitalization 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean APACHE II score on admission was 18.8 , the mean Charlson comorbidity index was 2.9 , and 20 ( 95.2 % ) patients had a history of intensive care unit hospitalization .
	manualset3
176427	1	410891	13	NULL	NULL	0	NULL	mean DNA content	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean DNA content of these two populations ( 0.067 and 0.131 microgram of DNA ) are approximately related by a factor of 2 .
	manualset3
176428	2	410891	13	NULL	NULL	0	NULL	two populations	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean DNA content of these two populations ( 0.067 and 0.131 microgram of DNA ) are approximately related by a factor of 2 .
	manualset3
176429	3	410891	13	NULL	NULL	0	NULL	 0.067 microgram	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean DNA content of these two populations ( 0.067 and 0.131 microgram of DNA ) are approximately related by a factor of 2 .
	manualset3
176430	4	410891	13	NULL	NULL	0	NULL	0.131 microgram 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean DNA content of these two populations ( 0.067 and 0.131 microgram of DNA ) are approximately related by a factor of 2 .
	manualset3
176431	5	410891	13	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean DNA content of these two populations ( 0.067 and 0.131 microgram of DNA ) are approximately related by a factor of 2 .
	manualset3
176432	6	410891	13	NULL	NULL	0	NULL	factor of 2 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean DNA content of these two populations ( 0.067 and 0.131 microgram of DNA ) are approximately related by a factor of 2 .
	manualset3
176433	1	410892	13	NULL	NULL	0	NULL	mean RBC/plasma concentration ratios	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean RBC/plasma concentration ratios were 23 , 61 , and 81 % for clozapine , N-desmethylclozapine , and clozapine N-oxide , respectively .
	manualset3
176434	2	410892	13	NULL	NULL	0	NULL	23 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean RBC/plasma concentration ratios were 23 , 61 , and 81 % for clozapine , N-desmethylclozapine , and clozapine N-oxide , respectively .
	manualset3
176435	3	410892	13	NULL	NULL	0	NULL	81 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean RBC/plasma concentration ratios were 23 , 61 , and 81 % for clozapine , N-desmethylclozapine , and clozapine N-oxide , respectively .
	manualset3
176436	4	410892	13	NULL	NULL	NULL	NULL	61 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The mean RBC/plasma concentration ratios were 23 , 61 , and 81 % for clozapine , N-desmethylclozapine , and clozapine N-oxide , respectively .
	manualset3
176437	5	410892	13	NULL	NULL	0	NULL	clozapine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean RBC/plasma concentration ratios were 23 , 61 , and 81 % for clozapine , N-desmethylclozapine , and clozapine N-oxide , respectively .
	manualset3
176438	6	410892	13	NULL	NULL	0	NULL	N-desmethylclozapine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean RBC/plasma concentration ratios were 23 , 61 , and 81 % for clozapine , N-desmethylclozapine , and clozapine N-oxide , respectively .
	manualset3
176439	7	410892	13	NULL	NULL	0	NULL	clozapine N-oxide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean RBC/plasma concentration ratios were 23 , 61 , and 81 % for clozapine , N-desmethylclozapine , and clozapine N-oxide , respectively .
	manualset3
176440	1	410893	13	NULL	NULL	0	NULL	mean SP	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean SP for all patients was 51 mm Hg .
	manualset3
176441	2	410893	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean SP for all patients was 51 mm Hg .
	manualset3
176442	3	410893	13	NULL	NULL	0	NULL	51 mm Hg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean SP for all patients was 51 mm Hg .
	manualset3
176443	1	410894	13	NULL	NULL	0	NULL	mean absolute recovery 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean absolute recovery for human serum was 101.7 + / - 6.1 % .
	manualset3
176444	2	410894	13	NULL	NULL	0	NULL	human serum	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean absolute recovery for human serum was 101.7 + / - 6.1 % .
	manualset3
176445	3	410894	13	NULL	NULL	0	NULL	101.7 + / - 6.1 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean absolute recovery for human serum was 101.7 + / - 6.1 % .
	manualset3
176446	1	410895	13	NULL	NULL	0	NULL	mean age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean age and prevalence of smoking , hypertension , diabetes mellitus , and hypercholesterolemia were not significantly different between 51 women with osteoporosis or osteopenia and 50 women with normal BMD .
	manualset3
176447	2	410895	13	NULL	NULL	0	NULL	prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean age and prevalence of smoking , hypertension , diabetes mellitus , and hypercholesterolemia were not significantly different between 51 women with osteoporosis or osteopenia and 50 women with normal BMD .
	manualset3
176448	3	410895	13	NULL	NULL	0	NULL	hypertension 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean age and prevalence of smoking , hypertension , diabetes mellitus , and hypercholesterolemia were not significantly different between 51 women with osteoporosis or osteopenia and 50 women with normal BMD .
	manualset3
176449	4	410895	13	NULL	NULL	0	NULL	 diabetes mellitus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean age and prevalence of smoking , hypertension , diabetes mellitus , and hypercholesterolemia were not significantly different between 51 women with osteoporosis or osteopenia and 50 women with normal BMD .
	manualset3
176450	5	410895	13	NULL	NULL	0	NULL	hypercholesterolemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean age and prevalence of smoking , hypertension , diabetes mellitus , and hypercholesterolemia were not significantly different between 51 women with osteoporosis or osteopenia and 50 women with normal BMD .
	manualset3
176451	6	410895	13	NULL	NULL	0	NULL	 51 women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean age and prevalence of smoking , hypertension , diabetes mellitus , and hypercholesterolemia were not significantly different between 51 women with osteoporosis or osteopenia and 50 women with normal BMD .
	manualset3
176452	7	410895	13	NULL	NULL	0	NULL	osteoporosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean age and prevalence of smoking , hypertension , diabetes mellitus , and hypercholesterolemia were not significantly different between 51 women with osteoporosis or osteopenia and 50 women with normal BMD .
	manualset3
176453	8	410895	13	NULL	NULL	0	NULL	osteopenia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean age and prevalence of smoking , hypertension , diabetes mellitus , and hypercholesterolemia were not significantly different between 51 women with osteoporosis or osteopenia and 50 women with normal BMD .
	manualset3
176454	9	410895	13	NULL	NULL	0	NULL	50 women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean age and prevalence of smoking , hypertension , diabetes mellitus , and hypercholesterolemia were not significantly different between 51 women with osteoporosis or osteopenia and 50 women with normal BMD .
	manualset3
176455	10	410895	13	NULL	NULL	0	NULL	normal BMD	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean age and prevalence of smoking , hypertension , diabetes mellitus , and hypercholesterolemia were not significantly different between 51 women with osteoporosis or osteopenia and 50 women with normal BMD .
	manualset3
176456	1	410896	13	NULL	NULL	0	NULL	mean antiproliferative effects	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean antiproliferative effects of IFN-gamma at 50 , 200 , and 500 U/ml for the PP group ( n = 10 ) was less compared to the NN group ( n = 11 ) ; P less than 0.001 , while the PN group ( n = 5 ) had a less dramatic , but statistically significant , reduction in growth inhibition by IFN-gamma only at 200 and 500 U/ml compared to NN cells ; P less than 0.05 and P less than 0.01 , respectively .
	manualset3
176457	2	410896	13	NULL	NULL	0	NULL	 IFN-gamma	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean antiproliferative effects of IFN-gamma at 50 , 200 , and 500 U/ml for the PP group ( n = 10 ) was less compared to the NN group ( n = 11 ) ; P less than 0.001 , while the PN group ( n = 5 ) had a less dramatic , but statistically significant , reduction in growth inhibition by IFN-gamma only at 200 and 500 U/ml compared to NN cells ; P less than 0.05 and P less than 0.01 , respectively .
	manualset3
176458	3	410896	13	NULL	NULL	0	NULL	50 U/ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean antiproliferative effects of IFN-gamma at 50 , 200 , and 500 U/ml for the PP group ( n = 10 ) was less compared to the NN group ( n = 11 ) ; P less than 0.001 , while the PN group ( n = 5 ) had a less dramatic , but statistically significant , reduction in growth inhibition by IFN-gamma only at 200 and 500 U/ml compared to NN cells ; P less than 0.05 and P less than 0.01 , respectively .
	manualset3
176459	4	410896	13	NULL	NULL	0	NULL	200 U/ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean antiproliferative effects of IFN-gamma at 50 , 200 , and 500 U/ml for the PP group ( n = 10 ) was less compared to the NN group ( n = 11 ) ; P less than 0.001 , while the PN group ( n = 5 ) had a less dramatic , but statistically significant , reduction in growth inhibition by IFN-gamma only at 200 and 500 U/ml compared to NN cells ; P less than 0.05 and P less than 0.01 , respectively .
	manualset3
176460	5	410896	13	NULL	NULL	0	NULL	500 U/ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean antiproliferative effects of IFN-gamma at 50 , 200 , and 500 U/ml for the PP group ( n = 10 ) was less compared to the NN group ( n = 11 ) ; P less than 0.001 , while the PN group ( n = 5 ) had a less dramatic , but statistically significant , reduction in growth inhibition by IFN-gamma only at 200 and 500 U/ml compared to NN cells ; P less than 0.05 and P less than 0.01 , respectively .
	manualset3
176461	6	410896	13	NULL	NULL	0	NULL	PP group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean antiproliferative effects of IFN-gamma at 50 , 200 , and 500 U/ml for the PP group ( n = 10 ) was less compared to the NN group ( n = 11 ) ; P less than 0.001 , while the PN group ( n = 5 ) had a less dramatic , but statistically significant , reduction in growth inhibition by IFN-gamma only at 200 and 500 U/ml compared to NN cells ; P less than 0.05 and P less than 0.01 , respectively .
	manualset3
176462	7	410896	13	NULL	NULL	0	NULL	n = 10 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean antiproliferative effects of IFN-gamma at 50 , 200 , and 500 U/ml for the PP group ( n = 10 ) was less compared to the NN group ( n = 11 ) ; P less than 0.001 , while the PN group ( n = 5 ) had a less dramatic , but statistically significant , reduction in growth inhibition by IFN-gamma only at 200 and 500 U/ml compared to NN cells ; P less than 0.05 and P less than 0.01 , respectively .
	manualset3
176463	8	410896	13	NULL	NULL	0	NULL	NN group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean antiproliferative effects of IFN-gamma at 50 , 200 , and 500 U/ml for the PP group ( n = 10 ) was less compared to the NN group ( n = 11 ) ; P less than 0.001 , while the PN group ( n = 5 ) had a less dramatic , but statistically significant , reduction in growth inhibition by IFN-gamma only at 200 and 500 U/ml compared to NN cells ; P less than 0.05 and P less than 0.01 , respectively .
	manualset3
176464	9	410896	13	NULL	NULL	0	NULL	n = 11	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean antiproliferative effects of IFN-gamma at 50 , 200 , and 500 U/ml for the PP group ( n = 10 ) was less compared to the NN group ( n = 11 ) ; P less than 0.001 , while the PN group ( n = 5 ) had a less dramatic , but statistically significant , reduction in growth inhibition by IFN-gamma only at 200 and 500 U/ml compared to NN cells ; P less than 0.05 and P less than 0.01 , respectively .
	manualset3
176465	10	410896	13	NULL	NULL	0	NULL	P less than 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean antiproliferative effects of IFN-gamma at 50 , 200 , and 500 U/ml for the PP group ( n = 10 ) was less compared to the NN group ( n = 11 ) ; P less than 0.001 , while the PN group ( n = 5 ) had a less dramatic , but statistically significant , reduction in growth inhibition by IFN-gamma only at 200 and 500 U/ml compared to NN cells ; P less than 0.05 and P less than 0.01 , respectively .
	manualset3
176466	11	410896	13	NULL	NULL	0	NULL	 PN group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean antiproliferative effects of IFN-gamma at 50 , 200 , and 500 U/ml for the PP group ( n = 10 ) was less compared to the NN group ( n = 11 ) ; P less than 0.001 , while the PN group ( n = 5 ) had a less dramatic , but statistically significant , reduction in growth inhibition by IFN-gamma only at 200 and 500 U/ml compared to NN cells ; P less than 0.05 and P less than 0.01 , respectively .
	manualset3
176467	12	410896	13	NULL	NULL	0	NULL	n = 5 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean antiproliferative effects of IFN-gamma at 50 , 200 , and 500 U/ml for the PP group ( n = 10 ) was less compared to the NN group ( n = 11 ) ; P less than 0.001 , while the PN group ( n = 5 ) had a less dramatic , but statistically significant , reduction in growth inhibition by IFN-gamma only at 200 and 500 U/ml compared to NN cells ; P less than 0.05 and P less than 0.01 , respectively .
	manualset3
176468	13	410896	13	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean antiproliferative effects of IFN-gamma at 50 , 200 , and 500 U/ml for the PP group ( n = 10 ) was less compared to the NN group ( n = 11 ) ; P less than 0.001 , while the PN group ( n = 5 ) had a less dramatic , but statistically significant , reduction in growth inhibition by IFN-gamma only at 200 and 500 U/ml compared to NN cells ; P less than 0.05 and P less than 0.01 , respectively .
	manualset3
176469	14	410896	13	NULL	NULL	0	NULL	growth inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean antiproliferative effects of IFN-gamma at 50 , 200 , and 500 U/ml for the PP group ( n = 10 ) was less compared to the NN group ( n = 11 ) ; P less than 0.001 , while the PN group ( n = 5 ) had a less dramatic , but statistically significant , reduction in growth inhibition by IFN-gamma only at 200 and 500 U/ml compared to NN cells ; P less than 0.05 and P less than 0.01 , respectively .
	manualset3
176470	15	410896	13	NULL	NULL	0	NULL	IFN-gamma	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean antiproliferative effects of IFN-gamma at 50 , 200 , and 500 U/ml for the PP group ( n = 10 ) was less compared to the NN group ( n = 11 ) ; P less than 0.001 , while the PN group ( n = 5 ) had a less dramatic , but statistically significant , reduction in growth inhibition by IFN-gamma only at 200 and 500 U/ml compared to NN cells ; P less than 0.05 and P less than 0.01 , respectively .
	manualset3
176471	16	410896	13	NULL	NULL	0	NULL	200 U/ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean antiproliferative effects of IFN-gamma at 50 , 200 , and 500 U/ml for the PP group ( n = 10 ) was less compared to the NN group ( n = 11 ) ; P less than 0.001 , while the PN group ( n = 5 ) had a less dramatic , but statistically significant , reduction in growth inhibition by IFN-gamma only at 200 and 500 U/ml compared to NN cells ; P less than 0.05 and P less than 0.01 , respectively .
	manualset3
176472	17	410896	13	NULL	NULL	0	NULL	500 U/ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean antiproliferative effects of IFN-gamma at 50 , 200 , and 500 U/ml for the PP group ( n = 10 ) was less compared to the NN group ( n = 11 ) ; P less than 0.001 , while the PN group ( n = 5 ) had a less dramatic , but statistically significant , reduction in growth inhibition by IFN-gamma only at 200 and 500 U/ml compared to NN cells ; P less than 0.05 and P less than 0.01 , respectively .
	manualset3
176473	18	410896	13	NULL	NULL	0	NULL	NN cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean antiproliferative effects of IFN-gamma at 50 , 200 , and 500 U/ml for the PP group ( n = 10 ) was less compared to the NN group ( n = 11 ) ; P less than 0.001 , while the PN group ( n = 5 ) had a less dramatic , but statistically significant , reduction in growth inhibition by IFN-gamma only at 200 and 500 U/ml compared to NN cells ; P less than 0.05 and P less than 0.01 , respectively .
	manualset3
176474	19	410896	13	NULL	NULL	0	NULL	P less than 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean antiproliferative effects of IFN-gamma at 50 , 200 , and 500 U/ml for the PP group ( n = 10 ) was less compared to the NN group ( n = 11 ) ; P less than 0.001 , while the PN group ( n = 5 ) had a less dramatic , but statistically significant , reduction in growth inhibition by IFN-gamma only at 200 and 500 U/ml compared to NN cells ; P less than 0.05 and P less than 0.01 , respectively .
	manualset3
176475	20	410896	13	NULL	NULL	0	NULL	P less than 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean antiproliferative effects of IFN-gamma at 50 , 200 , and 500 U/ml for the PP group ( n = 10 ) was less compared to the NN group ( n = 11 ) ; P less than 0.001 , while the PN group ( n = 5 ) had a less dramatic , but statistically significant , reduction in growth inhibition by IFN-gamma only at 200 and 500 U/ml compared to NN cells ; P less than 0.05 and P less than 0.01 , respectively .
	manualset3
176476	1	410897	13	NULL	NULL	0	NULL	mean barrier pressure 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean barrier pressure in the former group was significantly lower than the baseline for the 75 minutes studied .
	manualset3
176477	2	410897	13	NULL	NULL	0	NULL	 former group 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean barrier pressure in the former group was significantly lower than the baseline for the 75 minutes studied .
	manualset3
176478	3	410897	13	NULL	NULL	0	NULL	baseline	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean barrier pressure in the former group was significantly lower than the baseline for the 75 minutes studied .
	manualset3
176479	4	410897	13	NULL	NULL	0	NULL	75 minutes	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean barrier pressure in the former group was significantly lower than the baseline for the 75 minutes studied .
	manualset3
176480	1	410898	13	NULL	NULL	0	NULL	mean bile salt concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean bile salt concentration of those treated with Maalox ( 0.24 mM ) , Meciadanol ( 0.24 mM ) , or sucralfate ( 0.35 mM ) was significantly lower than those treated with nasogastric aspiration ( 0.87 mM ) alone ( P less than 0.01 ) .
	manualset3
176481	2	410898	13	NULL	NULL	0	NULL	Maalox 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean bile salt concentration of those treated with Maalox ( 0.24 mM ) , Meciadanol ( 0.24 mM ) , or sucralfate ( 0.35 mM ) was significantly lower than those treated with nasogastric aspiration ( 0.87 mM ) alone ( P less than 0.01 ) .
	manualset3
176482	3	410898	13	NULL	NULL	0	NULL	0.24 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean bile salt concentration of those treated with Maalox ( 0.24 mM ) , Meciadanol ( 0.24 mM ) , or sucralfate ( 0.35 mM ) was significantly lower than those treated with nasogastric aspiration ( 0.87 mM ) alone ( P less than 0.01 ) .
	manualset3
176483	4	410898	13	NULL	NULL	0	NULL	Meciadanol 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean bile salt concentration of those treated with Maalox ( 0.24 mM ) , Meciadanol ( 0.24 mM ) , or sucralfate ( 0.35 mM ) was significantly lower than those treated with nasogastric aspiration ( 0.87 mM ) alone ( P less than 0.01 ) .
	manualset3
176484	5	410898	13	NULL	NULL	0	NULL	0.24 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean bile salt concentration of those treated with Maalox ( 0.24 mM ) , Meciadanol ( 0.24 mM ) , or sucralfate ( 0.35 mM ) was significantly lower than those treated with nasogastric aspiration ( 0.87 mM ) alone ( P less than 0.01 ) .
	manualset3
176485	6	410898	13	NULL	NULL	0	NULL	sucralfate	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean bile salt concentration of those treated with Maalox ( 0.24 mM ) , Meciadanol ( 0.24 mM ) , or sucralfate ( 0.35 mM ) was significantly lower than those treated with nasogastric aspiration ( 0.87 mM ) alone ( P less than 0.01 ) .
	manualset3
176486	7	410898	13	NULL	NULL	0	NULL	0.35 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean bile salt concentration of those treated with Maalox ( 0.24 mM ) , Meciadanol ( 0.24 mM ) , or sucralfate ( 0.35 mM ) was significantly lower than those treated with nasogastric aspiration ( 0.87 mM ) alone ( P less than 0.01 ) .
	manualset3
176487	8	410898	13	NULL	NULL	0	NULL	nasogastric aspiration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean bile salt concentration of those treated with Maalox ( 0.24 mM ) , Meciadanol ( 0.24 mM ) , or sucralfate ( 0.35 mM ) was significantly lower than those treated with nasogastric aspiration ( 0.87 mM ) alone ( P less than 0.01 ) .
	manualset3
176488	9	410898	13	NULL	NULL	0	NULL	0.87 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean bile salt concentration of those treated with Maalox ( 0.24 mM ) , Meciadanol ( 0.24 mM ) , or sucralfate ( 0.35 mM ) was significantly lower than those treated with nasogastric aspiration ( 0.87 mM ) alone ( P less than 0.01 ) .
	manualset3
176489	10	410898	13	NULL	NULL	0	NULL	P less than 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean bile salt concentration of those treated with Maalox ( 0.24 mM ) , Meciadanol ( 0.24 mM ) , or sucralfate ( 0.35 mM ) was significantly lower than those treated with nasogastric aspiration ( 0.87 mM ) alone ( P less than 0.01 ) .
	manualset3
176490	1	410899	13	NULL	NULL	0	NULL	mean blood oxycodone concentration 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean blood oxycodone concentration was 0.40 mg/L ( range 0.06-53 .00 mg/L ) .
	manualset3
176491	2	410899	13	NULL	NULL	0	NULL	0.40 mg/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean blood oxycodone concentration was 0.40 mg/L ( range 0.06-53 .00 mg/L ) .
	manualset3
176492	3	410899	13	NULL	NULL	0	NULL	range 0.06-53 .00 mg/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean blood oxycodone concentration was 0.40 mg/L ( range 0.06-53 .00 mg/L ) .
	manualset3
176493	1	410900	13	NULL	NULL	0	NULL	mean concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean concentrations in liver and kidney were 500 + / -300 pg g ( -1 ) f.w. and 90 + / -50 pg g ( -1 ) f.w. , respectively .
	manualset3
176494	2	410900	13	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean concentrations in liver and kidney were 500 + / -300 pg g ( -1 ) f.w. and 90 + / -50 pg g ( -1 ) f.w. , respectively .
	manualset3
176495	3	410900	13	NULL	NULL	0	NULL	kidney	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean concentrations in liver and kidney were 500 + / -300 pg g ( -1 ) f.w. and 90 + / -50 pg g ( -1 ) f.w. , respectively .
	manualset3
176496	4	410900	13	NULL	NULL	0	NULL	500 + / -300 pg g ( -1 ) f.w. 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean concentrations in liver and kidney were 500 + / -300 pg g ( -1 ) f.w. and 90 + / -50 pg g ( -1 ) f.w. , respectively .
	manualset3
176497	5	410900	13	NULL	NULL	0	NULL	 90 + / -50 pg g ( -1 ) f.w. 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean concentrations in liver and kidney were 500 + / -300 pg g ( -1 ) f.w. and 90 + / -50 pg g ( -1 ) f.w. , respectively .
	manualset3
176498	1	410901	13	NULL	NULL	0	NULL	mean difference	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean difference in lipid area was 0.1 mm2 ( 95 % CI = -2.1 -2.3 mm2 ) .
	manualset3
176499	2	410901	13	NULL	NULL	0	NULL	lipid area	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean difference in lipid area was 0.1 mm2 ( 95 % CI = -2.1 -2.3 mm2 ) .
	manualset3
176500	3	410901	13	NULL	NULL	0	NULL	0.1 mm2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean difference in lipid area was 0.1 mm2 ( 95 % CI = -2.1 -2.3 mm2 ) .
	manualset3
176501	4	410901	13	NULL	NULL	0	NULL	95 % CI = -2.1 -2.3 mm2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean difference in lipid area was 0.1 mm2 ( 95 % CI = -2.1 -2.3 mm2 ) .
	manualset3
176502	1	410902	13	NULL	NULL	0	NULL	 mean distance	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean distance from the maxillary central incisor to the GPF was 57.58 mm .
	manualset3
176503	2	410902	13	NULL	NULL	0	NULL	maxillary central incisor	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean distance from the maxillary central incisor to the GPF was 57.58 mm .
	manualset3
176504	3	410902	13	NULL	NULL	0	NULL	GPF 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean distance from the maxillary central incisor to the GPF was 57.58 mm .
	manualset3
176505	4	410902	13	NULL	NULL	0	NULL	57.58 mm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean distance from the maxillary central incisor to the GPF was 57.58 mm .
	manualset3
176506	1	410903	13	NULL	NULL	0	NULL	trichromatic illuminant-object interaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A trichromatic illuminant-object interaction was simulated analogous to that resulting from illumination by three monochromatic lights .
	manualset3
176507	2	410903	13	NULL	NULL	0	NULL	illumination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A trichromatic illuminant-object interaction was simulated analogous to that resulting from illumination by three monochromatic lights .
	manualset3
176508	3	410903	13	NULL	NULL	0	NULL	three 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A trichromatic illuminant-object interaction was simulated analogous to that resulting from illumination by three monochromatic lights .
	manualset3
176509	4	410903	13	NULL	NULL	0	NULL	monochromatic lights 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	A trichromatic illuminant-object interaction was simulated analogous to that resulting from illumination by three monochromatic lights .
	manualset3
176510	1	410904	13	NULL	NULL	0	NULL	 mean half-life	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean half-life of hepatitis B immunoglobulin was calculated as 24.8 days , and in approximately 90 % of vaccines 300 , 000 mIU of hepatitis B immunoglobulin provided protection until an active immune response had developed .
	manualset3
176511	2	410904	13	NULL	NULL	0	NULL	hepatitis B immunoglobulin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean half-life of hepatitis B immunoglobulin was calculated as 24.8 days , and in approximately 90 % of vaccines 300 , 000 mIU of hepatitis B immunoglobulin provided protection until an active immune response had developed .
	manualset3
176512	3	410904	13	NULL	NULL	0	NULL	24.8 days 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean half-life of hepatitis B immunoglobulin was calculated as 24.8 days , and in approximately 90 % of vaccines 300 , 000 mIU of hepatitis B immunoglobulin provided protection until an active immune response had developed .
	manualset3
176513	4	410904	13	NULL	NULL	0	NULL	approximately 90 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean half-life of hepatitis B immunoglobulin was calculated as 24.8 days , and in approximately 90 % of vaccines 300 , 000 mIU of hepatitis B immunoglobulin provided protection until an active immune response had developed .
	manualset3
176514	5	410904	13	NULL	NULL	0	NULL	vaccines 300 , 000 mIU	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean half-life of hepatitis B immunoglobulin was calculated as 24.8 days , and in approximately 90 % of vaccines 300 , 000 mIU of hepatitis B immunoglobulin provided protection until an active immune response had developed .
	manualset3
176515	6	410904	13	NULL	NULL	0	NULL	hepatitis B immunoglobulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean half-life of hepatitis B immunoglobulin was calculated as 24.8 days , and in approximately 90 % of vaccines 300 , 000 mIU of hepatitis B immunoglobulin provided protection until an active immune response had developed .
	manualset3
176516	7	410904	13	NULL	NULL	0	NULL	protection 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean half-life of hepatitis B immunoglobulin was calculated as 24.8 days , and in approximately 90 % of vaccines 300 , 000 mIU of hepatitis B immunoglobulin provided protection until an active immune response had developed .
	manualset3
176517	8	410904	13	NULL	NULL	0	NULL	active immune response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean half-life of hepatitis B immunoglobulin was calculated as 24.8 days , and in approximately 90 % of vaccines 300 , 000 mIU of hepatitis B immunoglobulin provided protection until an active immune response had developed .
	manualset3
176518	1	410905	13	NULL	NULL	0	NULL	mean length	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean length of followup was 3.7 years .
	manualset3
176519	2	410905	13	NULL	NULL	0	NULL	followup 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean length of followup was 3.7 years .
	manualset3
176520	3	410905	13	NULL	NULL	0	NULL	3.7 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean length of followup was 3.7 years .
	manualset3
176521	1	410906	13	NULL	NULL	0	NULL	mean longevity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean longevity was 4.2 yr ; cows from the synthetic breed groups produced longer ( P & lt ; .01 ) than Hereford cows , due to a relatively faster rate of removal at all ages in the purebred Hereford group .
	manualset3
176522	2	410906	13	NULL	NULL	0	NULL	4.2 yr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean longevity was 4.2 yr ; cows from the synthetic breed groups produced longer ( P & lt ; .01 ) than Hereford cows , due to a relatively faster rate of removal at all ages in the purebred Hereford group .
	manualset3
176523	3	410906	13	NULL	NULL	0	NULL	cows 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean longevity was 4.2 yr ; cows from the synthetic breed groups produced longer ( P & lt ; .01 ) than Hereford cows , due to a relatively faster rate of removal at all ages in the purebred Hereford group .
	manualset3
176524	4	410906	13	NULL	NULL	0	NULL	 synthetic breed groups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean longevity was 4.2 yr ; cows from the synthetic breed groups produced longer ( P & lt ; .01 ) than Hereford cows , due to a relatively faster rate of removal at all ages in the purebred Hereford group .
	manualset3
176525	5	410906	13	NULL	NULL	0	NULL	P & lt ; .01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean longevity was 4.2 yr ; cows from the synthetic breed groups produced longer ( P & lt ; .01 ) than Hereford cows , due to a relatively faster rate of removal at all ages in the purebred Hereford group .
	manualset3
176526	6	410906	13	NULL	NULL	0	NULL	Hereford cows	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean longevity was 4.2 yr ; cows from the synthetic breed groups produced longer ( P & lt ; .01 ) than Hereford cows , due to a relatively faster rate of removal at all ages in the purebred Hereford group .
	manualset3
176527	7	410906	13	NULL	NULL	0	NULL	rate 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean longevity was 4.2 yr ; cows from the synthetic breed groups produced longer ( P & lt ; .01 ) than Hereford cows , due to a relatively faster rate of removal at all ages in the purebred Hereford group .
	manualset3
176528	8	410906	13	NULL	NULL	0	NULL	removal 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean longevity was 4.2 yr ; cows from the synthetic breed groups produced longer ( P & lt ; .01 ) than Hereford cows , due to a relatively faster rate of removal at all ages in the purebred Hereford group .
	manualset3
176529	9	410906	13	NULL	NULL	0	NULL	ages 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean longevity was 4.2 yr ; cows from the synthetic breed groups produced longer ( P & lt ; .01 ) than Hereford cows , due to a relatively faster rate of removal at all ages in the purebred Hereford group .
	manualset3
176530	10	410906	13	NULL	NULL	0	NULL	purebred Hereford group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean longevity was 4.2 yr ; cows from the synthetic breed groups produced longer ( P & lt ; .01 ) than Hereford cows , due to a relatively faster rate of removal at all ages in the purebred Hereford group .
	manualset3
176531	1	410907	13	NULL	NULL	0	NULL	mean 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean or alternatively the first PC ( PC ( 1 ) ) spectrum from the same region can be used for quantitation of peak areas of metabolites in the human brain at increased SNR .
	manualset3
176532	2	410907	13	NULL	NULL	0	NULL	first PC ( PC ( 1 ) ) spectrum	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean or alternatively the first PC ( PC ( 1 ) ) spectrum from the same region can be used for quantitation of peak areas of metabolites in the human brain at increased SNR .
	manualset3
176533	3	410907	13	NULL	NULL	0	NULL	same region 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean or alternatively the first PC ( PC ( 1 ) ) spectrum from the same region can be used for quantitation of peak areas of metabolites in the human brain at increased SNR .
	manualset3
176534	4	410907	13	NULL	NULL	0	NULL	 quantitation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean or alternatively the first PC ( PC ( 1 ) ) spectrum from the same region can be used for quantitation of peak areas of metabolites in the human brain at increased SNR .
	manualset3
176535	5	410907	13	NULL	NULL	0	NULL	peak areas	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean or alternatively the first PC ( PC ( 1 ) ) spectrum from the same region can be used for quantitation of peak areas of metabolites in the human brain at increased SNR .
	manualset3
176536	6	410907	13	NULL	NULL	0	NULL	metabolites 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean or alternatively the first PC ( PC ( 1 ) ) spectrum from the same region can be used for quantitation of peak areas of metabolites in the human brain at increased SNR .
	manualset3
176537	7	410907	13	NULL	NULL	0	NULL	human brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean or alternatively the first PC ( PC ( 1 ) ) spectrum from the same region can be used for quantitation of peak areas of metabolites in the human brain at increased SNR .
	manualset3
176538	8	410907	13	NULL	NULL	0	NULL	SNR	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean or alternatively the first PC ( PC ( 1 ) ) spectrum from the same region can be used for quantitation of peak areas of metabolites in the human brain at increased SNR .
	manualset3
176539	1	410908	13	NULL	NULL	0	NULL	mean percentage	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean percentage increase of FSH and LH was higher the greater the severity of liver cirrhosis .
	manualset3
176540	2	410908	13	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean percentage increase of FSH and LH was higher the greater the severity of liver cirrhosis .
	manualset3
176541	3	410908	13	NULL	NULL	0	NULL	FSH 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean percentage increase of FSH and LH was higher the greater the severity of liver cirrhosis .
	manualset3
176542	4	410908	13	NULL	NULL	0	NULL	LH 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean percentage increase of FSH and LH was higher the greater the severity of liver cirrhosis .
	manualset3
176543	5	410908	13	NULL	NULL	0	NULL	severity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean percentage increase of FSH and LH was higher the greater the severity of liver cirrhosis .
	manualset3
176544	6	410908	13	NULL	NULL	0	NULL	liver cirrhosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean percentage increase of FSH and LH was higher the greater the severity of liver cirrhosis .
	manualset3
176545	1	410909	13	NULL	NULL	0	NULL	 mean preoperative AOFAS score	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean preoperative AOFAS score was 52.0 + / - 16.8 .
	manualset3
176546	2	410909	13	NULL	NULL	0	NULL	 52.0 + / - 16.8	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean preoperative AOFAS score was 52.0 + / - 16.8 .
	manualset3
176547	1	410910	13	NULL	NULL	0	NULL	trigonometric series 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A trigonometric series is used to approximate the solution and the coefficients of the series as well as the duration of ejection and pre-ejection periods are chosen so that the governing differential equation is exactly satisfied at certain times during ejection ( the collocation points ) , as well as the boundary conditions and steady state condition .
	manualset3
176548	2	410910	13	NULL	NULL	0	NULL	solution 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A trigonometric series is used to approximate the solution and the coefficients of the series as well as the duration of ejection and pre-ejection periods are chosen so that the governing differential equation is exactly satisfied at certain times during ejection ( the collocation points ) , as well as the boundary conditions and steady state condition .
	manualset3
176549	3	410910	13	NULL	NULL	0	NULL	coefficients 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A trigonometric series is used to approximate the solution and the coefficients of the series as well as the duration of ejection and pre-ejection periods are chosen so that the governing differential equation is exactly satisfied at certain times during ejection ( the collocation points ) , as well as the boundary conditions and steady state condition .
	manualset3
176550	4	410910	13	NULL	NULL	0	NULL	series 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A trigonometric series is used to approximate the solution and the coefficients of the series as well as the duration of ejection and pre-ejection periods are chosen so that the governing differential equation is exactly satisfied at certain times during ejection ( the collocation points ) , as well as the boundary conditions and steady state condition .
	manualset3
176551	5	410910	13	NULL	NULL	0	NULL	duration 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A trigonometric series is used to approximate the solution and the coefficients of the series as well as the duration of ejection and pre-ejection periods are chosen so that the governing differential equation is exactly satisfied at certain times during ejection ( the collocation points ) , as well as the boundary conditions and steady state condition .
	manualset3
176552	6	410910	13	NULL	NULL	0	NULL	ejection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A trigonometric series is used to approximate the solution and the coefficients of the series as well as the duration of ejection and pre-ejection periods are chosen so that the governing differential equation is exactly satisfied at certain times during ejection ( the collocation points ) , as well as the boundary conditions and steady state condition .
	manualset3
176553	7	410910	13	NULL	NULL	0	NULL	pre-ejection periods 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A trigonometric series is used to approximate the solution and the coefficients of the series as well as the duration of ejection and pre-ejection periods are chosen so that the governing differential equation is exactly satisfied at certain times during ejection ( the collocation points ) , as well as the boundary conditions and steady state condition .
	manualset3
176554	8	410910	13	NULL	NULL	0	NULL	differential equation	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A trigonometric series is used to approximate the solution and the coefficients of the series as well as the duration of ejection and pre-ejection periods are chosen so that the governing differential equation is exactly satisfied at certain times during ejection ( the collocation points ) , as well as the boundary conditions and steady state condition .
	manualset3
176555	9	410910	13	NULL	NULL	0	NULL	times 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A trigonometric series is used to approximate the solution and the coefficients of the series as well as the duration of ejection and pre-ejection periods are chosen so that the governing differential equation is exactly satisfied at certain times during ejection ( the collocation points ) , as well as the boundary conditions and steady state condition .
	manualset3
176556	10	410910	13	NULL	NULL	0	NULL	 ejection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A trigonometric series is used to approximate the solution and the coefficients of the series as well as the duration of ejection and pre-ejection periods are chosen so that the governing differential equation is exactly satisfied at certain times during ejection ( the collocation points ) , as well as the boundary conditions and steady state condition .
	manualset3
176557	11	410910	13	NULL	NULL	0	NULL	collocation points	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A trigonometric series is used to approximate the solution and the coefficients of the series as well as the duration of ejection and pre-ejection periods are chosen so that the governing differential equation is exactly satisfied at certain times during ejection ( the collocation points ) , as well as the boundary conditions and steady state condition .
	manualset3
176558	12	410910	13	NULL	NULL	0	NULL	boundary conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A trigonometric series is used to approximate the solution and the coefficients of the series as well as the duration of ejection and pre-ejection periods are chosen so that the governing differential equation is exactly satisfied at certain times during ejection ( the collocation points ) , as well as the boundary conditions and steady state condition .
	manualset3
176559	13	410910	13	NULL	NULL	0	NULL	 steady state condition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A trigonometric series is used to approximate the solution and the coefficients of the series as well as the duration of ejection and pre-ejection periods are chosen so that the governing differential equation is exactly satisfied at certain times during ejection ( the collocation points ) , as well as the boundary conditions and steady state condition .
	manualset3
176560	1	410911	13	NULL	NULL	0	NULL	mean risk factor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean risk factor of all age groups shows a slight increase for carcinoma prevalence with 1 , 0 in P1 and N1 to approximately 1 , 5 in P2 ad 3 , 0 in Dy .
	manualset3
176561	2	410911	13	NULL	NULL	0	NULL	all age groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean risk factor of all age groups shows a slight increase for carcinoma prevalence with 1 , 0 in P1 and N1 to approximately 1 , 5 in P2 ad 3 , 0 in Dy .
	manualset3
176562	3	410911	13	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean risk factor of all age groups shows a slight increase for carcinoma prevalence with 1 , 0 in P1 and N1 to approximately 1 , 5 in P2 ad 3 , 0 in Dy .
	manualset3
176563	4	410911	13	NULL	NULL	0	NULL	carcinoma prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean risk factor of all age groups shows a slight increase for carcinoma prevalence with 1 , 0 in P1 and N1 to approximately 1 , 5 in P2 ad 3 , 0 in Dy .
	manualset3
176564	5	410911	13	NULL	NULL	0	NULL	1 , 0 in P1 and N1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean risk factor of all age groups shows a slight increase for carcinoma prevalence with 1 , 0 in P1 and N1 to approximately 1 , 5 in P2 ad 3 , 0 in Dy .
	manualset3
176565	6	410911	13	NULL	NULL	0	NULL	approximately 1 , 5 in P2 ad 3 , 0 in Dy	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean risk factor of all age groups shows a slight increase for carcinoma prevalence with 1 , 0 in P1 and N1 to approximately 1 , 5 in P2 ad 3 , 0 in Dy .
	manualset3
176566	1	410912	13	NULL	NULL	0	NULL	mean survival 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean survival was 31.2 and 15.6 months , respectively for patients with positive and negative endogenous estrogen .
	manualset3
176567	2	410912	13	NULL	NULL	0	NULL	31.2 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean survival was 31.2 and 15.6 months , respectively for patients with positive and negative endogenous estrogen .
	manualset3
176568	3	410912	13	NULL	NULL	0	NULL	15.6 months 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean survival was 31.2 and 15.6 months , respectively for patients with positive and negative endogenous estrogen .
	manualset3
176569	4	410912	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean survival was 31.2 and 15.6 months , respectively for patients with positive and negative endogenous estrogen .
	manualset3
176570	5	410912	13	NULL	NULL	0	NULL	positive endogenous estrogen	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean survival was 31.2 and 15.6 months , respectively for patients with positive and negative endogenous estrogen .
	manualset3
176571	6	410912	13	NULL	NULL	0	NULL	negative endogenous estrogen	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean survival was 31.2 and 15.6 months , respectively for patients with positive and negative endogenous estrogen .
	manualset3
176572	1	410913	13	NULL	NULL	0	NULL	mean time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean time of onset of epilepsy after central nervous system infection was 1.4 + / - 0.9 years ( range 0-19 years ) .
	manualset3
176573	2	410913	13	NULL	NULL	0	NULL	onset of epilepsy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean time of onset of epilepsy after central nervous system infection was 1.4 + / - 0.9 years ( range 0-19 years ) .
	manualset3
176574	3	410913	13	NULL	NULL	0	NULL	central nervous system infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean time of onset of epilepsy after central nervous system infection was 1.4 + / - 0.9 years ( range 0-19 years ) .
	manualset3
176575	4	410913	13	NULL	NULL	0	NULL	1.4 + / - 0.9 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean time of onset of epilepsy after central nervous system infection was 1.4 + / - 0.9 years ( range 0-19 years ) .
	manualset3
176576	5	410913	13	NULL	NULL	0	NULL	range 0-19 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean time of onset of epilepsy after central nervous system infection was 1.4 + / - 0.9 years ( range 0-19 years ) .
	manualset3
176577	1	410914	13	NULL	NULL	0	NULL	mean time period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean time period for sick leave was significantly shorter for group II , 6.5 + / - 1.6 weeks compared with 8.5 + / - 1.8 weeks for group I. The mean time period for return to sports activity was significantly shorter for group II , 9.5 + / - 2.2 weeks , compared with 12.5 + / - 2.6 weeks for group I. Early range of motion training is recommended after ligament reconstruction of the ankle , as it will enable earlier return to sports activities , shorter sick leave and preserved mechanical stability .
	manualset3
176578	2	410914	13	NULL	NULL	0	NULL	sick leave 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean time period for sick leave was significantly shorter for group II , 6.5 + / - 1.6 weeks compared with 8.5 + / - 1.8 weeks for group I. The mean time period for return to sports activity was significantly shorter for group II , 9.5 + / - 2.2 weeks , compared with 12.5 + / - 2.6 weeks for group I. Early range of motion training is recommended after ligament reconstruction of the ankle , as it will enable earlier return to sports activities , shorter sick leave and preserved mechanical stability .
	manualset3
176579	3	410914	13	NULL	NULL	0	NULL	group II	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean time period for sick leave was significantly shorter for group II , 6.5 + / - 1.6 weeks compared with 8.5 + / - 1.8 weeks for group I. The mean time period for return to sports activity was significantly shorter for group II , 9.5 + / - 2.2 weeks , compared with 12.5 + / - 2.6 weeks for group I. Early range of motion training is recommended after ligament reconstruction of the ankle , as it will enable earlier return to sports activities , shorter sick leave and preserved mechanical stability .
	manualset3
176580	4	410914	13	NULL	NULL	0	NULL	6.5 + / - 1.6 weeks 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean time period for sick leave was significantly shorter for group II , 6.5 + / - 1.6 weeks compared with 8.5 + / - 1.8 weeks for group I. The mean time period for return to sports activity was significantly shorter for group II , 9.5 + / - 2.2 weeks , compared with 12.5 + / - 2.6 weeks for group I. Early range of motion training is recommended after ligament reconstruction of the ankle , as it will enable earlier return to sports activities , shorter sick leave and preserved mechanical stability .
	manualset3
176581	5	410914	13	NULL	NULL	0	NULL	8.5 + / - 1.8 weeks 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean time period for sick leave was significantly shorter for group II , 6.5 + / - 1.6 weeks compared with 8.5 + / - 1.8 weeks for group I. The mean time period for return to sports activity was significantly shorter for group II , 9.5 + / - 2.2 weeks , compared with 12.5 + / - 2.6 weeks for group I. Early range of motion training is recommended after ligament reconstruction of the ankle , as it will enable earlier return to sports activities , shorter sick leave and preserved mechanical stability .
	manualset3
176582	6	410914	13	NULL	NULL	0	NULL	group I	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean time period for sick leave was significantly shorter for group II , 6.5 + / - 1.6 weeks compared with 8.5 + / - 1.8 weeks for group I. The mean time period for return to sports activity was significantly shorter for group II , 9.5 + / - 2.2 weeks , compared with 12.5 + / - 2.6 weeks for group I. Early range of motion training is recommended after ligament reconstruction of the ankle , as it will enable earlier return to sports activities , shorter sick leave and preserved mechanical stability .
	manualset3
176583	7	410914	13	NULL	NULL	0	NULL	mean time period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean time period for sick leave was significantly shorter for group II , 6.5 + / - 1.6 weeks compared with 8.5 + / - 1.8 weeks for group I. The mean time period for return to sports activity was significantly shorter for group II , 9.5 + / - 2.2 weeks , compared with 12.5 + / - 2.6 weeks for group I. Early range of motion training is recommended after ligament reconstruction of the ankle , as it will enable earlier return to sports activities , shorter sick leave and preserved mechanical stability .
	manualset3
176584	8	410914	13	NULL	NULL	0	NULL	sports activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean time period for sick leave was significantly shorter for group II , 6.5 + / - 1.6 weeks compared with 8.5 + / - 1.8 weeks for group I. The mean time period for return to sports activity was significantly shorter for group II , 9.5 + / - 2.2 weeks , compared with 12.5 + / - 2.6 weeks for group I. Early range of motion training is recommended after ligament reconstruction of the ankle , as it will enable earlier return to sports activities , shorter sick leave and preserved mechanical stability .
	manualset3
176585	9	410914	13	NULL	NULL	0	NULL	group II	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean time period for sick leave was significantly shorter for group II , 6.5 + / - 1.6 weeks compared with 8.5 + / - 1.8 weeks for group I. The mean time period for return to sports activity was significantly shorter for group II , 9.5 + / - 2.2 weeks , compared with 12.5 + / - 2.6 weeks for group I. Early range of motion training is recommended after ligament reconstruction of the ankle , as it will enable earlier return to sports activities , shorter sick leave and preserved mechanical stability .
	manualset3
176586	10	410914	13	NULL	NULL	0	NULL	9.5 + / - 2.2 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean time period for sick leave was significantly shorter for group II , 6.5 + / - 1.6 weeks compared with 8.5 + / - 1.8 weeks for group I. The mean time period for return to sports activity was significantly shorter for group II , 9.5 + / - 2.2 weeks , compared with 12.5 + / - 2.6 weeks for group I. Early range of motion training is recommended after ligament reconstruction of the ankle , as it will enable earlier return to sports activities , shorter sick leave and preserved mechanical stability .
	manualset3
176587	11	410914	13	NULL	NULL	0	NULL	12.5 + / - 2.6 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean time period for sick leave was significantly shorter for group II , 6.5 + / - 1.6 weeks compared with 8.5 + / - 1.8 weeks for group I. The mean time period for return to sports activity was significantly shorter for group II , 9.5 + / - 2.2 weeks , compared with 12.5 + / - 2.6 weeks for group I. Early range of motion training is recommended after ligament reconstruction of the ankle , as it will enable earlier return to sports activities , shorter sick leave and preserved mechanical stability .
	manualset3
176588	12	410914	13	NULL	NULL	0	NULL	group I	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean time period for sick leave was significantly shorter for group II , 6.5 + / - 1.6 weeks compared with 8.5 + / - 1.8 weeks for group I. The mean time period for return to sports activity was significantly shorter for group II , 9.5 + / - 2.2 weeks , compared with 12.5 + / - 2.6 weeks for group I. Early range of motion training is recommended after ligament reconstruction of the ankle , as it will enable earlier return to sports activities , shorter sick leave and preserved mechanical stability .
	manualset3
176589	13	410914	13	NULL	NULL	0	NULL	range	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean time period for sick leave was significantly shorter for group II , 6.5 + / - 1.6 weeks compared with 8.5 + / - 1.8 weeks for group I. The mean time period for return to sports activity was significantly shorter for group II , 9.5 + / - 2.2 weeks , compared with 12.5 + / - 2.6 weeks for group I. Early range of motion training is recommended after ligament reconstruction of the ankle , as it will enable earlier return to sports activities , shorter sick leave and preserved mechanical stability .
	manualset3
176590	14	410914	13	NULL	NULL	0	NULL	motion training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean time period for sick leave was significantly shorter for group II , 6.5 + / - 1.6 weeks compared with 8.5 + / - 1.8 weeks for group I. The mean time period for return to sports activity was significantly shorter for group II , 9.5 + / - 2.2 weeks , compared with 12.5 + / - 2.6 weeks for group I. Early range of motion training is recommended after ligament reconstruction of the ankle , as it will enable earlier return to sports activities , shorter sick leave and preserved mechanical stability .
	manualset3
176591	15	410914	13	NULL	NULL	0	NULL	ligament reconstruction 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean time period for sick leave was significantly shorter for group II , 6.5 + / - 1.6 weeks compared with 8.5 + / - 1.8 weeks for group I. The mean time period for return to sports activity was significantly shorter for group II , 9.5 + / - 2.2 weeks , compared with 12.5 + / - 2.6 weeks for group I. Early range of motion training is recommended after ligament reconstruction of the ankle , as it will enable earlier return to sports activities , shorter sick leave and preserved mechanical stability .
	manualset3
176592	16	410914	13	NULL	NULL	0	NULL	ankle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean time period for sick leave was significantly shorter for group II , 6.5 + / - 1.6 weeks compared with 8.5 + / - 1.8 weeks for group I. The mean time period for return to sports activity was significantly shorter for group II , 9.5 + / - 2.2 weeks , compared with 12.5 + / - 2.6 weeks for group I. Early range of motion training is recommended after ligament reconstruction of the ankle , as it will enable earlier return to sports activities , shorter sick leave and preserved mechanical stability .
	manualset3
176593	17	410914	13	NULL	NULL	0	NULL	sports activities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean time period for sick leave was significantly shorter for group II , 6.5 + / - 1.6 weeks compared with 8.5 + / - 1.8 weeks for group I. The mean time period for return to sports activity was significantly shorter for group II , 9.5 + / - 2.2 weeks , compared with 12.5 + / - 2.6 weeks for group I. Early range of motion training is recommended after ligament reconstruction of the ankle , as it will enable earlier return to sports activities , shorter sick leave and preserved mechanical stability .
	manualset3
176594	18	410914	13	NULL	NULL	0	NULL	sick leave	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean time period for sick leave was significantly shorter for group II , 6.5 + / - 1.6 weeks compared with 8.5 + / - 1.8 weeks for group I. The mean time period for return to sports activity was significantly shorter for group II , 9.5 + / - 2.2 weeks , compared with 12.5 + / - 2.6 weeks for group I. Early range of motion training is recommended after ligament reconstruction of the ankle , as it will enable earlier return to sports activities , shorter sick leave and preserved mechanical stability .
	manualset3
176595	19	410914	13	NULL	NULL	0	NULL	mechanical stability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean time period for sick leave was significantly shorter for group II , 6.5 + / - 1.6 weeks compared with 8.5 + / - 1.8 weeks for group I. The mean time period for return to sports activity was significantly shorter for group II , 9.5 + / - 2.2 weeks , compared with 12.5 + / - 2.6 weeks for group I. Early range of motion training is recommended after ligament reconstruction of the ankle , as it will enable earlier return to sports activities , shorter sick leave and preserved mechanical stability .
	manualset3
176596	1	410915	13	NULL	NULL	0	NULL	mean value	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean value of peripheral blood T lymphocyte response to PHA in untreated or treated patients was lower than that in healthy subjects .
	manualset3
176597	2	410915	13	NULL	NULL	0	NULL	peripheral blood T lymphocyte response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean value of peripheral blood T lymphocyte response to PHA in untreated or treated patients was lower than that in healthy subjects .
	manualset3
176598	3	410915	13	NULL	NULL	0	NULL	PHA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean value of peripheral blood T lymphocyte response to PHA in untreated or treated patients was lower than that in healthy subjects .
	manualset3
176599	4	410915	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean value of peripheral blood T lymphocyte response to PHA in untreated or treated patients was lower than that in healthy subjects .
	manualset3
176600	5	410915	13	NULL	NULL	0	NULL	healthy subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean value of peripheral blood T lymphocyte response to PHA in untreated or treated patients was lower than that in healthy subjects .
	manualset3
176601	1	410916	13	NULL	NULL	0	NULL	mean value	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean value of the free folate portion in legumes ( 73.1 % ) was comparable with the values of grain , cereal products and bakery products .
	manualset3
176602	2	410916	13	NULL	NULL	0	NULL	free folate portion	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean value of the free folate portion in legumes ( 73.1 % ) was comparable with the values of grain , cereal products and bakery products .
	manualset3
176603	3	410916	13	NULL	NULL	0	NULL	legumes	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean value of the free folate portion in legumes ( 73.1 % ) was comparable with the values of grain , cereal products and bakery products .
	manualset3
176604	4	410916	13	NULL	NULL	0	NULL	73.1 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean value of the free folate portion in legumes ( 73.1 % ) was comparable with the values of grain , cereal products and bakery products .
	manualset3
176605	5	410916	13	NULL	NULL	0	NULL	values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean value of the free folate portion in legumes ( 73.1 % ) was comparable with the values of grain , cereal products and bakery products .
	manualset3
176606	6	410916	13	NULL	NULL	0	NULL	 grain	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean value of the free folate portion in legumes ( 73.1 % ) was comparable with the values of grain , cereal products and bakery products .
	manualset3
176607	7	410916	13	NULL	NULL	0	NULL	cereal products	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean value of the free folate portion in legumes ( 73.1 % ) was comparable with the values of grain , cereal products and bakery products .
	manualset3
176608	8	410916	13	NULL	NULL	0	NULL	bakery products	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean value of the free folate portion in legumes ( 73.1 % ) was comparable with the values of grain , cereal products and bakery products .
	manualset3
176609	1	410917	13	NULL	NULL	0	NULL	trilateral approach 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A trilateral approach to the clinical management of chloroquine-induced pruritus among patients with malaria has been used .
	manualset3
176610	2	410917	13	NULL	NULL	0	NULL	clinical management 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A trilateral approach to the clinical management of chloroquine-induced pruritus among patients with malaria has been used .
	manualset3
176611	3	410917	13	NULL	NULL	0	NULL	 chloroquine-induced pruritus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A trilateral approach to the clinical management of chloroquine-induced pruritus among patients with malaria has been used .
	manualset3
176612	4	410917	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A trilateral approach to the clinical management of chloroquine-induced pruritus among patients with malaria has been used .
	manualset3
176613	5	410917	13	NULL	NULL	0	NULL	malaria	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A trilateral approach to the clinical management of chloroquine-induced pruritus among patients with malaria has been used .
	manualset3
176614	1	410918	13	NULL	NULL	NULL	NULL	mean + / - SD daily dose 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The mean + / - SD daily dose of olanzapine was 18.00 + / - 2.89 mg after 6 weeks of treatment .
	manualset3
176615	2	410918	13	NULL	NULL	0	NULL	olanzapine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean + / - SD daily dose of olanzapine was 18.00 + / - 2.89 mg after 6 weeks of treatment .
	manualset3
176616	3	410918	13	NULL	NULL	0	NULL	18.00 + / - 2.89 mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean + / - SD daily dose of olanzapine was 18.00 + / - 2.89 mg after 6 weeks of treatment .
	manualset3
176617	4	410918	13	NULL	NULL	0	NULL	6 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean + / - SD daily dose of olanzapine was 18.00 + / - 2.89 mg after 6 weeks of treatment .
	manualset3
176618	5	410918	13	NULL	NULL	0	NULL	 treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean + / - SD daily dose of olanzapine was 18.00 + / - 2.89 mg after 6 weeks of treatment .
	manualset3
176619	1	410919	13	NULL	NULL	0	NULL	mean + / - SD duration 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean + / - SD duration of employment as an inside attendant was 3.8 + / - 3.0 years ( range 1 - 9 years ) and the mean + / - SD number of hyperbaric exposures was 198 + / - 267 ( median 96 ; range 30 - 950 ) .
	manualset3
176620	2	410919	13	NULL	NULL	0	NULL	employment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean + / - SD duration of employment as an inside attendant was 3.8 + / - 3.0 years ( range 1 - 9 years ) and the mean + / - SD number of hyperbaric exposures was 198 + / - 267 ( median 96 ; range 30 - 950 ) .
	manualset3
176621	3	410919	13	NULL	NULL	0	NULL	attendant	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean + / - SD duration of employment as an inside attendant was 3.8 + / - 3.0 years ( range 1 - 9 years ) and the mean + / - SD number of hyperbaric exposures was 198 + / - 267 ( median 96 ; range 30 - 950 ) .
	manualset3
176622	4	410919	13	NULL	NULL	0	NULL	3.8 + / - 3.0 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean + / - SD duration of employment as an inside attendant was 3.8 + / - 3.0 years ( range 1 - 9 years ) and the mean + / - SD number of hyperbaric exposures was 198 + / - 267 ( median 96 ; range 30 - 950 ) .
	manualset3
176623	5	410919	13	NULL	NULL	0	NULL	range 1 - 9 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean + / - SD duration of employment as an inside attendant was 3.8 + / - 3.0 years ( range 1 - 9 years ) and the mean + / - SD number of hyperbaric exposures was 198 + / - 267 ( median 96 ; range 30 - 950 ) .
	manualset3
176624	6	410919	13	NULL	NULL	0	NULL	mean + / - SD number 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean + / - SD duration of employment as an inside attendant was 3.8 + / - 3.0 years ( range 1 - 9 years ) and the mean + / - SD number of hyperbaric exposures was 198 + / - 267 ( median 96 ; range 30 - 950 ) .
	manualset3
176625	7	410919	13	NULL	NULL	0	NULL	hyperbaric exposures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean + / - SD duration of employment as an inside attendant was 3.8 + / - 3.0 years ( range 1 - 9 years ) and the mean + / - SD number of hyperbaric exposures was 198 + / - 267 ( median 96 ; range 30 - 950 ) .
	manualset3
176626	8	410919	13	NULL	NULL	0	NULL	198 + / - 267 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean + / - SD duration of employment as an inside attendant was 3.8 + / - 3.0 years ( range 1 - 9 years ) and the mean + / - SD number of hyperbaric exposures was 198 + / - 267 ( median 96 ; range 30 - 950 ) .
	manualset3
176627	9	410919	13	NULL	NULL	0	NULL	median 96 ; range 30 - 950	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean + / - SD duration of employment as an inside attendant was 3.8 + / - 3.0 years ( range 1 - 9 years ) and the mean + / - SD number of hyperbaric exposures was 198 + / - 267 ( median 96 ; range 30 - 950 ) .
	manualset3
176628	1	410920	13	NULL	NULL	0	NULL	mean + / - SD levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean + / - SD levels in the benign tumor group ( 424 + / - 124 microM ) were significantly lower ( p less than 0.0004 ) than those in the reference group ( 642 + / - 195 microM ) .
	manualset3
176629	2	410920	13	NULL	NULL	0	NULL	benign tumor group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean + / - SD levels in the benign tumor group ( 424 + / - 124 microM ) were significantly lower ( p less than 0.0004 ) than those in the reference group ( 642 + / - 195 microM ) .
	manualset3
176630	3	410920	13	NULL	NULL	0	NULL	 424 + / - 124 microM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean + / - SD levels in the benign tumor group ( 424 + / - 124 microM ) were significantly lower ( p less than 0.0004 ) than those in the reference group ( 642 + / - 195 microM ) .
	manualset3
176631	4	410920	13	NULL	NULL	0	NULL	 p less than 0.0004 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean + / - SD levels in the benign tumor group ( 424 + / - 124 microM ) were significantly lower ( p less than 0.0004 ) than those in the reference group ( 642 + / - 195 microM ) .
	manualset3
176632	5	410920	13	NULL	NULL	0	NULL	reference group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean + / - SD levels in the benign tumor group ( 424 + / - 124 microM ) were significantly lower ( p less than 0.0004 ) than those in the reference group ( 642 + / - 195 microM ) .
	manualset3
176633	6	410920	13	NULL	NULL	0	NULL	642 + / - 195 microM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean + / - SD levels in the benign tumor group ( 424 + / - 124 microM ) were significantly lower ( p less than 0.0004 ) than those in the reference group ( 642 + / - 195 microM ) .
	manualset3
176634	1	410921	13	NULL	NULL	0	NULL	mean of healthy years	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean of healthy years increased during the period 1986-1990 by 1.09 % while equity adjusted healthy years ( HY ( EDE ) ) dropped by -1.78 % .
	manualset3
176635	2	410921	13	NULL	NULL	0	NULL	 period 1986-1990	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean of healthy years increased during the period 1986-1990 by 1.09 % while equity adjusted healthy years ( HY ( EDE ) ) dropped by -1.78 % .
	manualset3
176636	3	410921	13	NULL	NULL	0	NULL	1.09 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean of healthy years increased during the period 1986-1990 by 1.09 % while equity adjusted healthy years ( HY ( EDE ) ) dropped by -1.78 % .
	manualset3
176637	4	410921	13	NULL	NULL	0	NULL	equity 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean of healthy years increased during the period 1986-1990 by 1.09 % while equity adjusted healthy years ( HY ( EDE ) ) dropped by -1.78 % .
	manualset3
176638	5	410921	13	NULL	NULL	0	NULL	healthy years ( HY ( EDE ) ) 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean of healthy years increased during the period 1986-1990 by 1.09 % while equity adjusted healthy years ( HY ( EDE ) ) dropped by -1.78 % .
	manualset3
176639	6	410921	13	NULL	NULL	0	NULL	-1.78 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mean of healthy years increased during the period 1986-1990 by 1.09 % while equity adjusted healthy years ( HY ( EDE ) ) dropped by -1.78 % .
	manualset3
176640	1	410922	13	NULL	NULL	0	NULL	measles-mumps-rubella ( MMR ) vaccine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The measles-mumps-rubella ( MMR ) vaccine has been very effective in the elimination of disease and has high biosafety .
	manualset3
176641	2	410922	13	NULL	NULL	0	NULL	elimination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The measles-mumps-rubella ( MMR ) vaccine has been very effective in the elimination of disease and has high biosafety .
	manualset3
176642	3	410922	13	NULL	NULL	0	NULL	disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The measles-mumps-rubella ( MMR ) vaccine has been very effective in the elimination of disease and has high biosafety .
	manualset3
176643	4	410922	13	NULL	NULL	0	NULL	biosafety	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The measles-mumps-rubella ( MMR ) vaccine has been very effective in the elimination of disease and has high biosafety .
	manualset3
176644	1	410923	13	NULL	NULL	0	NULL	measure of contraction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The measure of contraction depends on the diagnosis ( TAO greater than ASO greater than DIA ) , on the age of patient and also the anatomical location of the artery in the case of TAO ( TP greater than greater than TA ) , on the associated hypertension in the case of ASO ( normotensive greater than hypertensive ) and finally on the time elapsed between the operation and usage of preparation if the agonist is KCl .
	manualset3
176645	2	410923	13	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The measure of contraction depends on the diagnosis ( TAO greater than ASO greater than DIA ) , on the age of patient and also the anatomical location of the artery in the case of TAO ( TP greater than greater than TA ) , on the associated hypertension in the case of ASO ( normotensive greater than hypertensive ) and finally on the time elapsed between the operation and usage of preparation if the agonist is KCl .
	manualset3
176646	3	410923	13	NULL	NULL	0	NULL	TAO	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The measure of contraction depends on the diagnosis ( TAO greater than ASO greater than DIA ) , on the age of patient and also the anatomical location of the artery in the case of TAO ( TP greater than greater than TA ) , on the associated hypertension in the case of ASO ( normotensive greater than hypertensive ) and finally on the time elapsed between the operation and usage of preparation if the agonist is KCl .
	manualset3
176647	4	410923	13	NULL	NULL	0	NULL	ASO 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The measure of contraction depends on the diagnosis ( TAO greater than ASO greater than DIA ) , on the age of patient and also the anatomical location of the artery in the case of TAO ( TP greater than greater than TA ) , on the associated hypertension in the case of ASO ( normotensive greater than hypertensive ) and finally on the time elapsed between the operation and usage of preparation if the agonist is KCl .
	manualset3
176648	5	410923	13	NULL	NULL	0	NULL	 DIA	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The measure of contraction depends on the diagnosis ( TAO greater than ASO greater than DIA ) , on the age of patient and also the anatomical location of the artery in the case of TAO ( TP greater than greater than TA ) , on the associated hypertension in the case of ASO ( normotensive greater than hypertensive ) and finally on the time elapsed between the operation and usage of preparation if the agonist is KCl .
	manualset3
176649	6	410923	13	NULL	NULL	0	NULL	age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The measure of contraction depends on the diagnosis ( TAO greater than ASO greater than DIA ) , on the age of patient and also the anatomical location of the artery in the case of TAO ( TP greater than greater than TA ) , on the associated hypertension in the case of ASO ( normotensive greater than hypertensive ) and finally on the time elapsed between the operation and usage of preparation if the agonist is KCl .
	manualset3
176650	7	410923	13	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The measure of contraction depends on the diagnosis ( TAO greater than ASO greater than DIA ) , on the age of patient and also the anatomical location of the artery in the case of TAO ( TP greater than greater than TA ) , on the associated hypertension in the case of ASO ( normotensive greater than hypertensive ) and finally on the time elapsed between the operation and usage of preparation if the agonist is KCl .
	manualset3
176651	8	410923	13	NULL	NULL	0	NULL	anatomical location	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The measure of contraction depends on the diagnosis ( TAO greater than ASO greater than DIA ) , on the age of patient and also the anatomical location of the artery in the case of TAO ( TP greater than greater than TA ) , on the associated hypertension in the case of ASO ( normotensive greater than hypertensive ) and finally on the time elapsed between the operation and usage of preparation if the agonist is KCl .
	manualset3
176652	9	410923	13	NULL	NULL	0	NULL	artery 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The measure of contraction depends on the diagnosis ( TAO greater than ASO greater than DIA ) , on the age of patient and also the anatomical location of the artery in the case of TAO ( TP greater than greater than TA ) , on the associated hypertension in the case of ASO ( normotensive greater than hypertensive ) and finally on the time elapsed between the operation and usage of preparation if the agonist is KCl .
	manualset3
176653	10	410923	13	NULL	NULL	0	NULL	case of TAO	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The measure of contraction depends on the diagnosis ( TAO greater than ASO greater than DIA ) , on the age of patient and also the anatomical location of the artery in the case of TAO ( TP greater than greater than TA ) , on the associated hypertension in the case of ASO ( normotensive greater than hypertensive ) and finally on the time elapsed between the operation and usage of preparation if the agonist is KCl .
	manualset3
176654	11	410923	13	NULL	NULL	0	NULL	TP 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The measure of contraction depends on the diagnosis ( TAO greater than ASO greater than DIA ) , on the age of patient and also the anatomical location of the artery in the case of TAO ( TP greater than greater than TA ) , on the associated hypertension in the case of ASO ( normotensive greater than hypertensive ) and finally on the time elapsed between the operation and usage of preparation if the agonist is KCl .
	manualset3
176655	12	410923	13	NULL	NULL	0	NULL	TA	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The measure of contraction depends on the diagnosis ( TAO greater than ASO greater than DIA ) , on the age of patient and also the anatomical location of the artery in the case of TAO ( TP greater than greater than TA ) , on the associated hypertension in the case of ASO ( normotensive greater than hypertensive ) and finally on the time elapsed between the operation and usage of preparation if the agonist is KCl .
	manualset3
176656	13	410923	13	NULL	NULL	0	NULL	hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The measure of contraction depends on the diagnosis ( TAO greater than ASO greater than DIA ) , on the age of patient and also the anatomical location of the artery in the case of TAO ( TP greater than greater than TA ) , on the associated hypertension in the case of ASO ( normotensive greater than hypertensive ) and finally on the time elapsed between the operation and usage of preparation if the agonist is KCl .
	manualset3
176657	14	410923	13	NULL	NULL	0	NULL	case of ASO	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The measure of contraction depends on the diagnosis ( TAO greater than ASO greater than DIA ) , on the age of patient and also the anatomical location of the artery in the case of TAO ( TP greater than greater than TA ) , on the associated hypertension in the case of ASO ( normotensive greater than hypertensive ) and finally on the time elapsed between the operation and usage of preparation if the agonist is KCl .
	manualset3
176658	15	410923	13	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The measure of contraction depends on the diagnosis ( TAO greater than ASO greater than DIA ) , on the age of patient and also the anatomical location of the artery in the case of TAO ( TP greater than greater than TA ) , on the associated hypertension in the case of ASO ( normotensive greater than hypertensive ) and finally on the time elapsed between the operation and usage of preparation if the agonist is KCl .
	manualset3
176659	16	410923	13	NULL	NULL	0	NULL	operation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The measure of contraction depends on the diagnosis ( TAO greater than ASO greater than DIA ) , on the age of patient and also the anatomical location of the artery in the case of TAO ( TP greater than greater than TA ) , on the associated hypertension in the case of ASO ( normotensive greater than hypertensive ) and finally on the time elapsed between the operation and usage of preparation if the agonist is KCl .
	manualset3
176660	17	410923	13	NULL	NULL	0	NULL	usage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The measure of contraction depends on the diagnosis ( TAO greater than ASO greater than DIA ) , on the age of patient and also the anatomical location of the artery in the case of TAO ( TP greater than greater than TA ) , on the associated hypertension in the case of ASO ( normotensive greater than hypertensive ) and finally on the time elapsed between the operation and usage of preparation if the agonist is KCl .
	manualset3
176661	18	410923	13	NULL	NULL	0	NULL	preparation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The measure of contraction depends on the diagnosis ( TAO greater than ASO greater than DIA ) , on the age of patient and also the anatomical location of the artery in the case of TAO ( TP greater than greater than TA ) , on the associated hypertension in the case of ASO ( normotensive greater than hypertensive ) and finally on the time elapsed between the operation and usage of preparation if the agonist is KCl .
	manualset3
176662	19	410923	13	NULL	NULL	0	NULL	 agonist	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The measure of contraction depends on the diagnosis ( TAO greater than ASO greater than DIA ) , on the age of patient and also the anatomical location of the artery in the case of TAO ( TP greater than greater than TA ) , on the associated hypertension in the case of ASO ( normotensive greater than hypertensive ) and finally on the time elapsed between the operation and usage of preparation if the agonist is KCl .
	manualset3
176663	20	410923	13	NULL	NULL	0	NULL	KCl 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The measure of contraction depends on the diagnosis ( TAO greater than ASO greater than DIA ) , on the age of patient and also the anatomical location of the artery in the case of TAO ( TP greater than greater than TA ) , on the associated hypertension in the case of ASO ( normotensive greater than hypertensive ) and finally on the time elapsed between the operation and usage of preparation if the agonist is KCl .
	manualset3
176664	1	410924	13	NULL	NULL	0	NULL	magnetization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The measured magnetization is associated with structural defects formed at the interfaces of nanocrystals in their films , and discussed in terms of the defect-related itinerant-electron-mediated mechanism .
	manualset3
176665	2	410924	13	NULL	NULL	0	NULL	defects 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The measured magnetization is associated with structural defects formed at the interfaces of nanocrystals in their films , and discussed in terms of the defect-related itinerant-electron-mediated mechanism .
	manualset3
176666	3	410924	13	NULL	NULL	0	NULL	interfaces	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The measured magnetization is associated with structural defects formed at the interfaces of nanocrystals in their films , and discussed in terms of the defect-related itinerant-electron-mediated mechanism .
	manualset3
176667	4	410924	13	NULL	NULL	0	NULL	nanocrystals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The measured magnetization is associated with structural defects formed at the interfaces of nanocrystals in their films , and discussed in terms of the defect-related itinerant-electron-mediated mechanism .
	manualset3
176668	5	410924	13	NULL	NULL	0	NULL	films 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The measured magnetization is associated with structural defects formed at the interfaces of nanocrystals in their films , and discussed in terms of the defect-related itinerant-electron-mediated mechanism .
	manualset3
176669	6	410924	13	NULL	NULL	0	NULL	terms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The measured magnetization is associated with structural defects formed at the interfaces of nanocrystals in their films , and discussed in terms of the defect-related itinerant-electron-mediated mechanism .
	manualset3
176670	7	410924	13	NULL	NULL	0	NULL	 mechanism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The measured magnetization is associated with structural defects formed at the interfaces of nanocrystals in their films , and discussed in terms of the defect-related itinerant-electron-mediated mechanism .
	manualset3
176671	1	410925	13	NULL	NULL	0	NULL	 measurement 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurement is based on quantifying the lateral force required to induce the maximal deflection of the nanowire where the AFM tip was scanning over the surface in contact mode .
	manualset3
176672	2	410925	13	NULL	NULL	0	NULL	lateral force	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurement is based on quantifying the lateral force required to induce the maximal deflection of the nanowire where the AFM tip was scanning over the surface in contact mode .
	manualset3
176673	3	410925	13	NULL	NULL	0	NULL	deflection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurement is based on quantifying the lateral force required to induce the maximal deflection of the nanowire where the AFM tip was scanning over the surface in contact mode .
	manualset3
176674	4	410925	13	NULL	NULL	0	NULL	nanowire 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurement is based on quantifying the lateral force required to induce the maximal deflection of the nanowire where the AFM tip was scanning over the surface in contact mode .
	manualset3
176675	5	410925	13	NULL	NULL	0	NULL	AFM tip	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurement is based on quantifying the lateral force required to induce the maximal deflection of the nanowire where the AFM tip was scanning over the surface in contact mode .
	manualset3
176676	6	410925	13	NULL	NULL	0	NULL	surface	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurement is based on quantifying the lateral force required to induce the maximal deflection of the nanowire where the AFM tip was scanning over the surface in contact mode .
	manualset3
176677	7	410925	13	NULL	NULL	0	NULL	contact mode	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurement is based on quantifying the lateral force required to induce the maximal deflection of the nanowire where the AFM tip was scanning over the surface in contact mode .
	manualset3
176678	1	410926	13	NULL	NULL	0	NULL	measurement 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurement of RA flare is composed of data collection assessing a range of unique domains describing key features of RA worsening at the time of patient self-report of flare , and then periodically for the duration of the flare .
	manualset3
176679	2	410926	13	NULL	NULL	0	NULL	RA flare 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurement of RA flare is composed of data collection assessing a range of unique domains describing key features of RA worsening at the time of patient self-report of flare , and then periodically for the duration of the flare .
	manualset3
176680	3	410926	13	NULL	NULL	0	NULL	data collection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurement of RA flare is composed of data collection assessing a range of unique domains describing key features of RA worsening at the time of patient self-report of flare , and then periodically for the duration of the flare .
	manualset3
176681	4	410926	13	NULL	NULL	0	NULL	range	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurement of RA flare is composed of data collection assessing a range of unique domains describing key features of RA worsening at the time of patient self-report of flare , and then periodically for the duration of the flare .
	manualset3
176682	5	410926	13	NULL	NULL	0	NULL	unique domains	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurement of RA flare is composed of data collection assessing a range of unique domains describing key features of RA worsening at the time of patient self-report of flare , and then periodically for the duration of the flare .
	manualset3
176683	6	410926	13	NULL	NULL	0	NULL	key features 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurement of RA flare is composed of data collection assessing a range of unique domains describing key features of RA worsening at the time of patient self-report of flare , and then periodically for the duration of the flare .
	manualset3
176684	7	410926	13	NULL	NULL	0	NULL	RA	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurement of RA flare is composed of data collection assessing a range of unique domains describing key features of RA worsening at the time of patient self-report of flare , and then periodically for the duration of the flare .
	manualset3
176685	8	410926	13	NULL	NULL	0	NULL	worsening 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurement of RA flare is composed of data collection assessing a range of unique domains describing key features of RA worsening at the time of patient self-report of flare , and then periodically for the duration of the flare .
	manualset3
176686	9	410926	13	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurement of RA flare is composed of data collection assessing a range of unique domains describing key features of RA worsening at the time of patient self-report of flare , and then periodically for the duration of the flare .
	manualset3
176687	10	410926	13	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurement of RA flare is composed of data collection assessing a range of unique domains describing key features of RA worsening at the time of patient self-report of flare , and then periodically for the duration of the flare .
	manualset3
176688	11	410926	13	NULL	NULL	0	NULL	flare	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurement of RA flare is composed of data collection assessing a range of unique domains describing key features of RA worsening at the time of patient self-report of flare , and then periodically for the duration of the flare .
	manualset3
176689	12	410926	13	NULL	NULL	0	NULL	duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurement of RA flare is composed of data collection assessing a range of unique domains describing key features of RA worsening at the time of patient self-report of flare , and then periodically for the duration of the flare .
	manualset3
176690	13	410926	13	NULL	NULL	0	NULL	flare	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurement of RA flare is composed of data collection assessing a range of unique domains describing key features of RA worsening at the time of patient self-report of flare , and then periodically for the duration of the flare .
	manualset3
176691	1	410927	13	NULL	NULL	0	NULL	measurements 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurements in the presence and absence of labelled/cold L-leucine allowed the estimation of L-leucine levels and radioactivity by using a simple set of calculations and a standard curve built with known cold L-leucine concentrations in the presence of a fixed known amount of ( 14C ) L-leucine .
	manualset3
176692	2	410927	13	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurements in the presence and absence of labelled/cold L-leucine allowed the estimation of L-leucine levels and radioactivity by using a simple set of calculations and a standard curve built with known cold L-leucine concentrations in the presence of a fixed known amount of ( 14C ) L-leucine .
	manualset3
176693	3	410927	13	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurements in the presence and absence of labelled/cold L-leucine allowed the estimation of L-leucine levels and radioactivity by using a simple set of calculations and a standard curve built with known cold L-leucine concentrations in the presence of a fixed known amount of ( 14C ) L-leucine .
	manualset3
176694	4	410927	13	NULL	NULL	0	NULL	L-leucine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurements in the presence and absence of labelled/cold L-leucine allowed the estimation of L-leucine levels and radioactivity by using a simple set of calculations and a standard curve built with known cold L-leucine concentrations in the presence of a fixed known amount of ( 14C ) L-leucine .
	manualset3
176695	5	410927	13	NULL	NULL	0	NULL	estimation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurements in the presence and absence of labelled/cold L-leucine allowed the estimation of L-leucine levels and radioactivity by using a simple set of calculations and a standard curve built with known cold L-leucine concentrations in the presence of a fixed known amount of ( 14C ) L-leucine .
	manualset3
176696	6	410927	13	NULL	NULL	0	NULL	L-leucine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurements in the presence and absence of labelled/cold L-leucine allowed the estimation of L-leucine levels and radioactivity by using a simple set of calculations and a standard curve built with known cold L-leucine concentrations in the presence of a fixed known amount of ( 14C ) L-leucine .
	manualset3
176697	7	410927	13	NULL	NULL	0	NULL	levels 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurements in the presence and absence of labelled/cold L-leucine allowed the estimation of L-leucine levels and radioactivity by using a simple set of calculations and a standard curve built with known cold L-leucine concentrations in the presence of a fixed known amount of ( 14C ) L-leucine .
	manualset3
176698	8	410927	13	NULL	NULL	0	NULL	radioactivity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurements in the presence and absence of labelled/cold L-leucine allowed the estimation of L-leucine levels and radioactivity by using a simple set of calculations and a standard curve built with known cold L-leucine concentrations in the presence of a fixed known amount of ( 14C ) L-leucine .
	manualset3
176699	9	410927	13	NULL	NULL	0	NULL	simple set 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurements in the presence and absence of labelled/cold L-leucine allowed the estimation of L-leucine levels and radioactivity by using a simple set of calculations and a standard curve built with known cold L-leucine concentrations in the presence of a fixed known amount of ( 14C ) L-leucine .
	manualset3
176700	10	410927	13	NULL	NULL	0	NULL	calculations 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurements in the presence and absence of labelled/cold L-leucine allowed the estimation of L-leucine levels and radioactivity by using a simple set of calculations and a standard curve built with known cold L-leucine concentrations in the presence of a fixed known amount of ( 14C ) L-leucine .
	manualset3
176701	11	410927	13	NULL	NULL	0	NULL	standard curve	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurements in the presence and absence of labelled/cold L-leucine allowed the estimation of L-leucine levels and radioactivity by using a simple set of calculations and a standard curve built with known cold L-leucine concentrations in the presence of a fixed known amount of ( 14C ) L-leucine .
	manualset3
176702	12	410927	13	NULL	NULL	0	NULL	L-leucine 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurements in the presence and absence of labelled/cold L-leucine allowed the estimation of L-leucine levels and radioactivity by using a simple set of calculations and a standard curve built with known cold L-leucine concentrations in the presence of a fixed known amount of ( 14C ) L-leucine .
	manualset3
176703	13	410927	13	NULL	NULL	0	NULL	concentrations 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurements in the presence and absence of labelled/cold L-leucine allowed the estimation of L-leucine levels and radioactivity by using a simple set of calculations and a standard curve built with known cold L-leucine concentrations in the presence of a fixed known amount of ( 14C ) L-leucine .
	manualset3
176704	14	410927	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurements in the presence and absence of labelled/cold L-leucine allowed the estimation of L-leucine levels and radioactivity by using a simple set of calculations and a standard curve built with known cold L-leucine concentrations in the presence of a fixed known amount of ( 14C ) L-leucine .
	manualset3
176705	15	410927	13	NULL	NULL	0	NULL	amount 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurements in the presence and absence of labelled/cold L-leucine allowed the estimation of L-leucine levels and radioactivity by using a simple set of calculations and a standard curve built with known cold L-leucine concentrations in the presence of a fixed known amount of ( 14C ) L-leucine .
	manualset3
176706	16	410927	13	NULL	NULL	0	NULL	( 14C ) L-leucine 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The measurements in the presence and absence of labelled/cold L-leucine allowed the estimation of L-leucine levels and radioactivity by using a simple set of calculations and a standard curve built with known cold L-leucine concentrations in the presence of a fixed known amount of ( 14C ) L-leucine .
	manualset3
176707	1	410928	13	NULL	NULL	NULL	NULL	trilayer tubular scaffold 	Thing												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A trilayer tubular scaffold was fabricated by sequential electrospinning of blends of elastin/gelatin , PDS/elastin/gelatin , and PDS/gelatin ( EG/PEG/PG ) to mimic the complex matrix structure of native arteries .
	manualset3
176708	2	410928	13	NULL	NULL	0	NULL	electrospinning 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A trilayer tubular scaffold was fabricated by sequential electrospinning of blends of elastin/gelatin , PDS/elastin/gelatin , and PDS/gelatin ( EG/PEG/PG ) to mimic the complex matrix structure of native arteries .
	manualset3
176709	3	410928	13	NULL	NULL	0	NULL	blends 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A trilayer tubular scaffold was fabricated by sequential electrospinning of blends of elastin/gelatin , PDS/elastin/gelatin , and PDS/gelatin ( EG/PEG/PG ) to mimic the complex matrix structure of native arteries .
	manualset3
176710	4	410928	13	NULL	NULL	0	NULL	elastin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A trilayer tubular scaffold was fabricated by sequential electrospinning of blends of elastin/gelatin , PDS/elastin/gelatin , and PDS/gelatin ( EG/PEG/PG ) to mimic the complex matrix structure of native arteries .
	manualset3
176711	5	410928	13	NULL	NULL	NULL	NULL	gelatin 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A trilayer tubular scaffold was fabricated by sequential electrospinning of blends of elastin/gelatin , PDS/elastin/gelatin , and PDS/gelatin ( EG/PEG/PG ) to mimic the complex matrix structure of native arteries .
	manualset3
176712	6	410928	13	NULL	NULL	0	NULL	PDS	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A trilayer tubular scaffold was fabricated by sequential electrospinning of blends of elastin/gelatin , PDS/elastin/gelatin , and PDS/gelatin ( EG/PEG/PG ) to mimic the complex matrix structure of native arteries .
	manualset3
176713	7	410928	13	NULL	NULL	0	NULL	elastin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A trilayer tubular scaffold was fabricated by sequential electrospinning of blends of elastin/gelatin , PDS/elastin/gelatin , and PDS/gelatin ( EG/PEG/PG ) to mimic the complex matrix structure of native arteries .
	manualset3
176714	8	410928	13	NULL	NULL	0	NULL	gelatin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A trilayer tubular scaffold was fabricated by sequential electrospinning of blends of elastin/gelatin , PDS/elastin/gelatin , and PDS/gelatin ( EG/PEG/PG ) to mimic the complex matrix structure of native arteries .
	manualset3
176715	9	410928	13	NULL	NULL	0	NULL	PDS	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A trilayer tubular scaffold was fabricated by sequential electrospinning of blends of elastin/gelatin , PDS/elastin/gelatin , and PDS/gelatin ( EG/PEG/PG ) to mimic the complex matrix structure of native arteries .
	manualset3
176716	10	410928	13	NULL	NULL	0	NULL	gelatin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A trilayer tubular scaffold was fabricated by sequential electrospinning of blends of elastin/gelatin , PDS/elastin/gelatin , and PDS/gelatin ( EG/PEG/PG ) to mimic the complex matrix structure of native arteries .
	manualset3
176717	11	410928	13	NULL	NULL	0	NULL	EG	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A trilayer tubular scaffold was fabricated by sequential electrospinning of blends of elastin/gelatin , PDS/elastin/gelatin , and PDS/gelatin ( EG/PEG/PG ) to mimic the complex matrix structure of native arteries .
	manualset3
176718	12	410928	13	NULL	NULL	0	NULL	PEG	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A trilayer tubular scaffold was fabricated by sequential electrospinning of blends of elastin/gelatin , PDS/elastin/gelatin , and PDS/gelatin ( EG/PEG/PG ) to mimic the complex matrix structure of native arteries .
	manualset3
176719	13	410928	13	NULL	NULL	0	NULL	PG	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A trilayer tubular scaffold was fabricated by sequential electrospinning of blends of elastin/gelatin , PDS/elastin/gelatin , and PDS/gelatin ( EG/PEG/PG ) to mimic the complex matrix structure of native arteries .
	manualset3
176720	14	410928	13	NULL	NULL	0	NULL	complex matrix structure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A trilayer tubular scaffold was fabricated by sequential electrospinning of blends of elastin/gelatin , PDS/elastin/gelatin , and PDS/gelatin ( EG/PEG/PG ) to mimic the complex matrix structure of native arteries .
	manualset3
176721	15	410928	13	NULL	NULL	0	NULL	arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A trilayer tubular scaffold was fabricated by sequential electrospinning of blends of elastin/gelatin , PDS/elastin/gelatin , and PDS/gelatin ( EG/PEG/PG ) to mimic the complex matrix structure of native arteries .
	manualset3
176722	1	410929	13	NULL	NULL	0	NULL	catheter	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The measuring catheter is advanced across the pulmonary valve into the PA. .
	manualset3
176723	2	410929	13	NULL	NULL	0	NULL	pulmonary valve 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The measuring catheter is advanced across the pulmonary valve into the PA. .
	manualset3
176724	3	410929	13	NULL	NULL	0	NULL	PA	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The measuring catheter is advanced across the pulmonary valve into the PA. .
	manualset3
176725	1	410930	13	NULL	NULL	0	NULL	mechanism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism , diagnosis and prevention results and means ) .
	manualset3
176726	2	410930	13	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism , diagnosis and prevention results and means ) .
	manualset3
176727	3	410930	13	NULL	NULL	0	NULL	prevention 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism , diagnosis and prevention results and means ) .
	manualset3
176728	4	410930	13	NULL	NULL	0	NULL	results 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism , diagnosis and prevention results and means ) .
	manualset3
176729	5	410930	13	NULL	NULL	0	NULL	means 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism , diagnosis and prevention results and means ) .
	manualset3
176730	1	410931	13	NULL	NULL	0	NULL	mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism is mainly dependent on the PI3K protein .
	manualset3
176731	2	410931	13	NULL	NULL	0	NULL	PI3K protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism is mainly dependent on the PI3K protein .
	manualset3
176732	1	410932	13	NULL	NULL	0	NULL	mechanism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism of photochemical grafting of alkenes to H-terminated silicon has remained poorly understood .
	manualset3
176733	2	410932	13	NULL	NULL	0	NULL	photochemical grafting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism of photochemical grafting of alkenes to H-terminated silicon has remained poorly understood .
	manualset3
176734	3	410932	13	NULL	NULL	0	NULL	alkenes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism of photochemical grafting of alkenes to H-terminated silicon has remained poorly understood .
	manualset3
176735	4	410932	13	NULL	NULL	0	NULL	 H-terminated silicon 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism of photochemical grafting of alkenes to H-terminated silicon has remained poorly understood .
	manualset3
176736	1	410933	13	NULL	NULL	0	NULL	mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism of the effect of insulin on pyruvate kinase was not established .
	manualset3
176737	2	410933	13	NULL	NULL	0	NULL	effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism of the effect of insulin on pyruvate kinase was not established .
	manualset3
176738	3	410933	13	NULL	NULL	0	NULL	insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism of the effect of insulin on pyruvate kinase was not established .
	manualset3
176739	4	410933	13	NULL	NULL	0	NULL	pyruvate kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism of the effect of insulin on pyruvate kinase was not established .
	manualset3
176740	1	410934	13	NULL	NULL	0	NULL	 mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism of the heart 's adaption to prolonged load and dynamics of RNA synthesis in the myocardium .
	manualset3
176741	2	410934	13	NULL	NULL	0	NULL	 heart 's adaption 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism of the heart 's adaption to prolonged load and dynamics of RNA synthesis in the myocardium .
	manualset3
176742	3	410934	13	NULL	NULL	0	NULL	load	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism of the heart 's adaption to prolonged load and dynamics of RNA synthesis in the myocardium .
	manualset3
176743	4	410934	13	NULL	NULL	0	NULL	dynamics	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism of the heart 's adaption to prolonged load and dynamics of RNA synthesis in the myocardium .
	manualset3
176744	5	410934	13	NULL	NULL	0	NULL	RNA synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism of the heart 's adaption to prolonged load and dynamics of RNA synthesis in the myocardium .
	manualset3
176745	6	410934	13	NULL	NULL	0	NULL	myocardium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism of the heart 's adaption to prolonged load and dynamics of RNA synthesis in the myocardium .
	manualset3
176746	1	410935	13	NULL	NULL	0	NULL	mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism of the transport of phosphate in the intestine is via a proton symporter whilst in the parotid gland it is effected by a Na + coupled transporter .
	manualset3
176747	2	410935	13	NULL	NULL	0	NULL	transport	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism of the transport of phosphate in the intestine is via a proton symporter whilst in the parotid gland it is effected by a Na + coupled transporter .
	manualset3
176748	3	410935	13	NULL	NULL	0	NULL	phosphate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism of the transport of phosphate in the intestine is via a proton symporter whilst in the parotid gland it is effected by a Na + coupled transporter .
	manualset3
176749	4	410935	13	NULL	NULL	0	NULL	intestine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism of the transport of phosphate in the intestine is via a proton symporter whilst in the parotid gland it is effected by a Na + coupled transporter .
	manualset3
176750	5	410935	13	NULL	NULL	0	NULL	 proton symporter whilst	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism of the transport of phosphate in the intestine is via a proton symporter whilst in the parotid gland it is effected by a Na + coupled transporter .
	manualset3
176751	6	410935	13	NULL	NULL	0	NULL	 parotid gland	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism of the transport of phosphate in the intestine is via a proton symporter whilst in the parotid gland it is effected by a Na + coupled transporter .
	manualset3
176752	7	410935	13	NULL	NULL	0	NULL	Na + coupled transporter 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism of the transport of phosphate in the intestine is via a proton symporter whilst in the parotid gland it is effected by a Na + coupled transporter .
	manualset3
176753	1	410936	13	NULL	NULL	0	NULL	mechanism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism underlying this increased sensitivity of Pglyrp2 ( - / - ) mice to 12-O-tetradecanoylphorbol 13-acetate-induced psoriasis-like inflammation is reduced recruitment of regulatory T cells to the skin and enhanced production and activation of Th17 cells in the skin in Pglyrp2 ( - / - ) mice , which results in more severe inflammation and keratinocyte proliferation .
	manualset3
176754	2	410936	13	NULL	NULL	0	NULL	sensitivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism underlying this increased sensitivity of Pglyrp2 ( - / - ) mice to 12-O-tetradecanoylphorbol 13-acetate-induced psoriasis-like inflammation is reduced recruitment of regulatory T cells to the skin and enhanced production and activation of Th17 cells in the skin in Pglyrp2 ( - / - ) mice , which results in more severe inflammation and keratinocyte proliferation .
	manualset3
176755	3	410936	13	NULL	NULL	0	NULL	Pglyrp2 ( - / - ) mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism underlying this increased sensitivity of Pglyrp2 ( - / - ) mice to 12-O-tetradecanoylphorbol 13-acetate-induced psoriasis-like inflammation is reduced recruitment of regulatory T cells to the skin and enhanced production and activation of Th17 cells in the skin in Pglyrp2 ( - / - ) mice , which results in more severe inflammation and keratinocyte proliferation .
	manualset3
176756	4	410936	13	NULL	NULL	0	NULL	12-O-tetradecanoylphorbol 13-acetate-induced psoriasis-like inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism underlying this increased sensitivity of Pglyrp2 ( - / - ) mice to 12-O-tetradecanoylphorbol 13-acetate-induced psoriasis-like inflammation is reduced recruitment of regulatory T cells to the skin and enhanced production and activation of Th17 cells in the skin in Pglyrp2 ( - / - ) mice , which results in more severe inflammation and keratinocyte proliferation .
	manualset3
176757	5	410936	13	NULL	NULL	0	NULL	recruitment	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism underlying this increased sensitivity of Pglyrp2 ( - / - ) mice to 12-O-tetradecanoylphorbol 13-acetate-induced psoriasis-like inflammation is reduced recruitment of regulatory T cells to the skin and enhanced production and activation of Th17 cells in the skin in Pglyrp2 ( - / - ) mice , which results in more severe inflammation and keratinocyte proliferation .
	manualset3
176758	6	410936	13	NULL	NULL	0	NULL	regulatory T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism underlying this increased sensitivity of Pglyrp2 ( - / - ) mice to 12-O-tetradecanoylphorbol 13-acetate-induced psoriasis-like inflammation is reduced recruitment of regulatory T cells to the skin and enhanced production and activation of Th17 cells in the skin in Pglyrp2 ( - / - ) mice , which results in more severe inflammation and keratinocyte proliferation .
	manualset3
176759	7	410936	13	NULL	NULL	0	NULL	skin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism underlying this increased sensitivity of Pglyrp2 ( - / - ) mice to 12-O-tetradecanoylphorbol 13-acetate-induced psoriasis-like inflammation is reduced recruitment of regulatory T cells to the skin and enhanced production and activation of Th17 cells in the skin in Pglyrp2 ( - / - ) mice , which results in more severe inflammation and keratinocyte proliferation .
	manualset3
176760	8	410936	13	NULL	NULL	0	NULL	production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism underlying this increased sensitivity of Pglyrp2 ( - / - ) mice to 12-O-tetradecanoylphorbol 13-acetate-induced psoriasis-like inflammation is reduced recruitment of regulatory T cells to the skin and enhanced production and activation of Th17 cells in the skin in Pglyrp2 ( - / - ) mice , which results in more severe inflammation and keratinocyte proliferation .
	manualset3
176761	9	410936	13	NULL	NULL	0	NULL	activation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism underlying this increased sensitivity of Pglyrp2 ( - / - ) mice to 12-O-tetradecanoylphorbol 13-acetate-induced psoriasis-like inflammation is reduced recruitment of regulatory T cells to the skin and enhanced production and activation of Th17 cells in the skin in Pglyrp2 ( - / - ) mice , which results in more severe inflammation and keratinocyte proliferation .
	manualset3
176762	10	410936	13	NULL	NULL	0	NULL	Th17 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism underlying this increased sensitivity of Pglyrp2 ( - / - ) mice to 12-O-tetradecanoylphorbol 13-acetate-induced psoriasis-like inflammation is reduced recruitment of regulatory T cells to the skin and enhanced production and activation of Th17 cells in the skin in Pglyrp2 ( - / - ) mice , which results in more severe inflammation and keratinocyte proliferation .
	manualset3
176763	11	410936	13	NULL	NULL	0	NULL	skin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism underlying this increased sensitivity of Pglyrp2 ( - / - ) mice to 12-O-tetradecanoylphorbol 13-acetate-induced psoriasis-like inflammation is reduced recruitment of regulatory T cells to the skin and enhanced production and activation of Th17 cells in the skin in Pglyrp2 ( - / - ) mice , which results in more severe inflammation and keratinocyte proliferation .
	manualset3
176764	12	410936	13	NULL	NULL	0	NULL	 Pglyrp2 ( - / - ) mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism underlying this increased sensitivity of Pglyrp2 ( - / - ) mice to 12-O-tetradecanoylphorbol 13-acetate-induced psoriasis-like inflammation is reduced recruitment of regulatory T cells to the skin and enhanced production and activation of Th17 cells in the skin in Pglyrp2 ( - / - ) mice , which results in more severe inflammation and keratinocyte proliferation .
	manualset3
176765	13	410936	13	NULL	NULL	0	NULL	severe inflammation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism underlying this increased sensitivity of Pglyrp2 ( - / - ) mice to 12-O-tetradecanoylphorbol 13-acetate-induced psoriasis-like inflammation is reduced recruitment of regulatory T cells to the skin and enhanced production and activation of Th17 cells in the skin in Pglyrp2 ( - / - ) mice , which results in more severe inflammation and keratinocyte proliferation .
	manualset3
176766	14	410936	13	NULL	NULL	0	NULL	keratinocyte proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism underlying this increased sensitivity of Pglyrp2 ( - / - ) mice to 12-O-tetradecanoylphorbol 13-acetate-induced psoriasis-like inflammation is reduced recruitment of regulatory T cells to the skin and enhanced production and activation of Th17 cells in the skin in Pglyrp2 ( - / - ) mice , which results in more severe inflammation and keratinocyte proliferation .
	manualset3
176767	1	410937	13	NULL	NULL	0	NULL	triple-lumen perfusion technique	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A triple-lumen perfusion technique was employed ; the test solutions were isotonic and contained 0 , 5 , 10 , 25 , 40 , or 50 mM of a SCFA as the sodium salt .
	manualset3
176768	2	410937	13	NULL	NULL	0	NULL	test solutions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A triple-lumen perfusion technique was employed ; the test solutions were isotonic and contained 0 , 5 , 10 , 25 , 40 , or 50 mM of a SCFA as the sodium salt .
	manualset3
176769	3	410937	13	NULL	NULL	0	NULL	0 mM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A triple-lumen perfusion technique was employed ; the test solutions were isotonic and contained 0 , 5 , 10 , 25 , 40 , or 50 mM of a SCFA as the sodium salt .
	manualset3
176770	4	410937	13	NULL	NULL	0	NULL	5 mM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A triple-lumen perfusion technique was employed ; the test solutions were isotonic and contained 0 , 5 , 10 , 25 , 40 , or 50 mM of a SCFA as the sodium salt .
	manualset3
176771	5	410937	13	NULL	NULL	0	NULL	10 mM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A triple-lumen perfusion technique was employed ; the test solutions were isotonic and contained 0 , 5 , 10 , 25 , 40 , or 50 mM of a SCFA as the sodium salt .
	manualset3
176772	6	410937	13	NULL	NULL	0	NULL	25 mM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A triple-lumen perfusion technique was employed ; the test solutions were isotonic and contained 0 , 5 , 10 , 25 , 40 , or 50 mM of a SCFA as the sodium salt .
	manualset3
176773	7	410937	13	NULL	NULL	0	NULL	40 mM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A triple-lumen perfusion technique was employed ; the test solutions were isotonic and contained 0 , 5 , 10 , 25 , 40 , or 50 mM of a SCFA as the sodium salt .
	manualset3
176774	8	410937	13	NULL	NULL	0	NULL	50 mM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A triple-lumen perfusion technique was employed ; the test solutions were isotonic and contained 0 , 5 , 10 , 25 , 40 , or 50 mM of a SCFA as the sodium salt .
	manualset3
176775	9	410937	13	NULL	NULL	0	NULL	SCFA	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A triple-lumen perfusion technique was employed ; the test solutions were isotonic and contained 0 , 5 , 10 , 25 , 40 , or 50 mM of a SCFA as the sodium salt .
	manualset3
176776	10	410937	13	NULL	NULL	0	NULL	sodium salt 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A triple-lumen perfusion technique was employed ; the test solutions were isotonic and contained 0 , 5 , 10 , 25 , 40 , or 50 mM of a SCFA as the sodium salt .
	manualset3
176777	1	410938	13	NULL	NULL	0	NULL	 mechanism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism with three paths to products is of special interest because the effects of cooperativity can be studied .
	manualset3
176778	2	410938	13	NULL	NULL	0	NULL	three paths	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism with three paths to products is of special interest because the effects of cooperativity can be studied .
	manualset3
176779	3	410938	13	NULL	NULL	0	NULL	 interest 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism with three paths to products is of special interest because the effects of cooperativity can be studied .
	manualset3
176780	4	410938	13	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism with three paths to products is of special interest because the effects of cooperativity can be studied .
	manualset3
176781	5	410938	13	NULL	NULL	0	NULL	cooperativity	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanism with three paths to products is of special interest because the effects of cooperativity can be studied .
	manualset3
176782	1	410939	13	NULL	NULL	0	NULL	mechanisms 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanisms involved in DNA electrotransfer , which include cell electropermeabilization and DNA electrophoresis , are also surveyed .
	manualset3
176783	2	410939	13	NULL	NULL	0	NULL	DNA electrotransfer 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanisms involved in DNA electrotransfer , which include cell electropermeabilization and DNA electrophoresis , are also surveyed .
	manualset3
176784	3	410939	13	NULL	NULL	NULL	NULL	cell electropermeabilization 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The mechanisms involved in DNA electrotransfer , which include cell electropermeabilization and DNA electrophoresis , are also surveyed .
	manualset3
176785	4	410939	13	NULL	NULL	0	NULL	DNA electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanisms involved in DNA electrotransfer , which include cell electropermeabilization and DNA electrophoresis , are also surveyed .
	manualset3
176786	1	410940	13	NULL	NULL	NULL	NULL	 mechanisms	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The mechanisms of incorporation of two antigens have been determined using a monoclonal antibody ( 3A10 ) raised against the material released from the mycelial cell wall by zymolyase digestion and retained on a concanavalin A column .
	manualset3
176787	2	410940	13	NULL	NULL	0	NULL	incorporation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanisms of incorporation of two antigens have been determined using a monoclonal antibody ( 3A10 ) raised against the material released from the mycelial cell wall by zymolyase digestion and retained on a concanavalin A column .
	manualset3
176788	3	410940	13	NULL	NULL	0	NULL	two antigens	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanisms of incorporation of two antigens have been determined using a monoclonal antibody ( 3A10 ) raised against the material released from the mycelial cell wall by zymolyase digestion and retained on a concanavalin A column .
	manualset3
176789	4	410940	13	NULL	NULL	0	NULL	monoclonal antibody ( 3A10 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanisms of incorporation of two antigens have been determined using a monoclonal antibody ( 3A10 ) raised against the material released from the mycelial cell wall by zymolyase digestion and retained on a concanavalin A column .
	manualset3
176790	5	410940	13	NULL	NULL	0	NULL	material 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanisms of incorporation of two antigens have been determined using a monoclonal antibody ( 3A10 ) raised against the material released from the mycelial cell wall by zymolyase digestion and retained on a concanavalin A column .
	manualset3
176791	6	410940	13	NULL	NULL	0	NULL	mycelial cell wall	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanisms of incorporation of two antigens have been determined using a monoclonal antibody ( 3A10 ) raised against the material released from the mycelial cell wall by zymolyase digestion and retained on a concanavalin A column .
	manualset3
176792	7	410940	13	NULL	NULL	0	NULL	 zymolyase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanisms of incorporation of two antigens have been determined using a monoclonal antibody ( 3A10 ) raised against the material released from the mycelial cell wall by zymolyase digestion and retained on a concanavalin A column .
	manualset3
176793	8	410940	13	NULL	NULL	0	NULL	digestion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mechanisms of incorporation of two antigens have been determined using a monoclonal antibody ( 3A10 ) raised against the material released from the mycelial cell wall by zymolyase digestion and retained on a concanavalin A column .
	manualset3
176794	9	410940	13	NULL	NULL	NULL	NULL	concanavalin A column	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The mechanisms of incorporation of two antigens have been determined using a monoclonal antibody ( 3A10 ) raised against the material released from the mycelial cell wall by zymolyase digestion and retained on a concanavalin A column .
	manualset3
176795	1	410941	13	NULL	NULL	0	NULL	median PZ levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The median PZ levels in patients with HELLP syndrome were found to be significantly lower than those of pregnant women .
	manualset3
176796	2	410941	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The median PZ levels in patients with HELLP syndrome were found to be significantly lower than those of pregnant women .
	manualset3
176797	3	410941	13	NULL	NULL	0	NULL	HELLP syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The median PZ levels in patients with HELLP syndrome were found to be significantly lower than those of pregnant women .
	manualset3
176798	4	410941	13	NULL	NULL	0	NULL	pregnant women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The median PZ levels in patients with HELLP syndrome were found to be significantly lower than those of pregnant women .
	manualset3
176799	1	410942	13	NULL	NULL	0	NULL	median age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The median age of decreased patients ( group A ) was 60.5 years at the time of arteriography and of patients alive after follow-up ( group B ) 55.5 years , respectively ( p = 0.007 ) .
	manualset3
176800	2	410942	13	NULL	NULL	0	NULL	patients ( group A ) 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The median age of decreased patients ( group A ) was 60.5 years at the time of arteriography and of patients alive after follow-up ( group B ) 55.5 years , respectively ( p = 0.007 ) .
	manualset3
176801	3	410942	13	NULL	NULL	0	NULL	60.5 years	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The median age of decreased patients ( group A ) was 60.5 years at the time of arteriography and of patients alive after follow-up ( group B ) 55.5 years , respectively ( p = 0.007 ) .
	manualset3
176802	4	410942	13	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The median age of decreased patients ( group A ) was 60.5 years at the time of arteriography and of patients alive after follow-up ( group B ) 55.5 years , respectively ( p = 0.007 ) .
	manualset3
176803	5	410942	13	NULL	NULL	0	NULL	arteriography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The median age of decreased patients ( group A ) was 60.5 years at the time of arteriography and of patients alive after follow-up ( group B ) 55.5 years , respectively ( p = 0.007 ) .
	manualset3
176804	6	410942	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The median age of decreased patients ( group A ) was 60.5 years at the time of arteriography and of patients alive after follow-up ( group B ) 55.5 years , respectively ( p = 0.007 ) .
	manualset3
176805	7	410942	13	NULL	NULL	0	NULL	follow-up 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The median age of decreased patients ( group A ) was 60.5 years at the time of arteriography and of patients alive after follow-up ( group B ) 55.5 years , respectively ( p = 0.007 ) .
	manualset3
176806	8	410942	13	NULL	NULL	0	NULL	group B	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The median age of decreased patients ( group A ) was 60.5 years at the time of arteriography and of patients alive after follow-up ( group B ) 55.5 years , respectively ( p = 0.007 ) .
	manualset3
176807	9	410942	13	NULL	NULL	0	NULL	 55.5 years	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The median age of decreased patients ( group A ) was 60.5 years at the time of arteriography and of patients alive after follow-up ( group B ) 55.5 years , respectively ( p = 0.007 ) .
	manualset3
176808	10	410942	13	NULL	NULL	0	NULL	p = 0.007 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The median age of decreased patients ( group A ) was 60.5 years at the time of arteriography and of patients alive after follow-up ( group B ) 55.5 years , respectively ( p = 0.007 ) .
	manualset3
176809	1	410943	13	NULL	NULL	0	NULL	median effect concentration ( EC50 ) 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The median effect concentration ( EC50 ) of REE was 24.1 , 41.6-73 .8 and 55.3-150 .1 mg x kg ( -1 ) for soil bacteria , actinomycetes and fungi , respectively .
	manualset3
176810	2	410943	13	NULL	NULL	0	NULL	REE 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The median effect concentration ( EC50 ) of REE was 24.1 , 41.6-73 .8 and 55.3-150 .1 mg x kg ( -1 ) for soil bacteria , actinomycetes and fungi , respectively .
	manualset3
176811	3	410943	13	NULL	NULL	0	NULL	24.1 mg x kg ( -1 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The median effect concentration ( EC50 ) of REE was 24.1 , 41.6-73 .8 and 55.3-150 .1 mg x kg ( -1 ) for soil bacteria , actinomycetes and fungi , respectively .
	manualset3
176812	4	410943	13	NULL	NULL	0	NULL	41.6-73 .8 mg x kg ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The median effect concentration ( EC50 ) of REE was 24.1 , 41.6-73 .8 and 55.3-150 .1 mg x kg ( -1 ) for soil bacteria , actinomycetes and fungi , respectively .
	manualset3
176813	5	410943	13	NULL	NULL	0	NULL	55.3-150 .1 mg x kg ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The median effect concentration ( EC50 ) of REE was 24.1 , 41.6-73 .8 and 55.3-150 .1 mg x kg ( -1 ) for soil bacteria , actinomycetes and fungi , respectively .
	manualset3
176814	6	410943	13	NULL	NULL	0	NULL	soil bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The median effect concentration ( EC50 ) of REE was 24.1 , 41.6-73 .8 and 55.3-150 .1 mg x kg ( -1 ) for soil bacteria , actinomycetes and fungi , respectively .
	manualset3
176815	7	410943	13	NULL	NULL	0	NULL	actinomycetes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The median effect concentration ( EC50 ) of REE was 24.1 , 41.6-73 .8 and 55.3-150 .1 mg x kg ( -1 ) for soil bacteria , actinomycetes and fungi , respectively .
	manualset3
176816	8	410943	13	NULL	NULL	0	NULL	fungi	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The median effect concentration ( EC50 ) of REE was 24.1 , 41.6-73 .8 and 55.3-150 .1 mg x kg ( -1 ) for soil bacteria , actinomycetes and fungi , respectively .
	manualset3
176817	1	410944	13	NULL	NULL	0	NULL	cel5Z gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A truncated cel5Z gene was constructed with the addition of a nonsense mutation that removes the C-terminal region of the protein .
	manualset3
176818	2	410944	13	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A truncated cel5Z gene was constructed with the addition of a nonsense mutation that removes the C-terminal region of the protein .
	manualset3
176819	3	410944	13	NULL	NULL	0	NULL	nonsense mutation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A truncated cel5Z gene was constructed with the addition of a nonsense mutation that removes the C-terminal region of the protein .
	manualset3
176820	4	410944	13	NULL	NULL	0	NULL	C-terminal region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A truncated cel5Z gene was constructed with the addition of a nonsense mutation that removes the C-terminal region of the protein .
	manualset3
176821	5	410944	13	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A truncated cel5Z gene was constructed with the addition of a nonsense mutation that removes the C-terminal region of the protein .
	manualset3
176822	1	410945	13	NULL	NULL	0	NULL	median peripheral blood CD34 ( + ) cell count	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The median peripheral blood CD34 ( + ) cell count on day 5 of G-CSF was 21 cells/microl ( range 10-40 cells/microl ) .
	manualset3
176823	2	410945	13	NULL	NULL	0	NULL	day 5	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The median peripheral blood CD34 ( + ) cell count on day 5 of G-CSF was 21 cells/microl ( range 10-40 cells/microl ) .
	manualset3
176824	3	410945	13	NULL	NULL	0	NULL	G-CSF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The median peripheral blood CD34 ( + ) cell count on day 5 of G-CSF was 21 cells/microl ( range 10-40 cells/microl ) .
	manualset3
176825	4	410945	13	NULL	NULL	NULL	NULL	21 cells/microl 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The median peripheral blood CD34 ( + ) cell count on day 5 of G-CSF was 21 cells/microl ( range 10-40 cells/microl ) .
	manualset3
176826	5	410945	13	NULL	NULL	0	NULL	range 10-40 cells/microl 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The median peripheral blood CD34 ( + ) cell count on day 5 of G-CSF was 21 cells/microl ( range 10-40 cells/microl ) .
	manualset3
176827	1	410946	13	NULL	NULL	0	NULL	median time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The median time of recovery to WHO grade 0 was 62 and 128 days , respectively .
	manualset3
176828	2	410946	13	NULL	NULL	0	NULL	recovery	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The median time of recovery to WHO grade 0 was 62 and 128 days , respectively .
	manualset3
176829	3	410946	13	NULL	NULL	0	NULL	WHO grade 0 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The median time of recovery to WHO grade 0 was 62 and 128 days , respectively .
	manualset3
176830	4	410946	13	NULL	NULL	0	NULL	62 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The median time of recovery to WHO grade 0 was 62 and 128 days , respectively .
	manualset3
176831	5	410946	13	NULL	NULL	0	NULL	128 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The median time of recovery to WHO grade 0 was 62 and 128 days , respectively .
	manualset3
176832	1	410947	13	NULL	NULL	0	NULL	median time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The median time to HCMV reactivation was 54 days ( range , 16-245 days ) after NST .
	manualset3
176833	2	410947	13	NULL	NULL	0	NULL	HCMV reactivation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The median time to HCMV reactivation was 54 days ( range , 16-245 days ) after NST .
	manualset3
176834	3	410947	13	NULL	NULL	0	NULL	54 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The median time to HCMV reactivation was 54 days ( range , 16-245 days ) after NST .
	manualset3
176835	4	410947	13	NULL	NULL	0	NULL	range , 16-245 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The median time to HCMV reactivation was 54 days ( range , 16-245 days ) after NST .
	manualset3
176836	5	410947	13	NULL	NULL	0	NULL	NST	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The median time to HCMV reactivation was 54 days ( range , 16-245 days ) after NST .
	manualset3
176837	1	410948	13	NULL	NULL	0	NULL	median time to disease progression ( TTP )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The median time to disease progression ( TTP ) was 251 days and 252 days for anastrozole and tamoxifen , respectively .
	manualset3
176838	2	410948	13	NULL	NULL	0	NULL	251 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The median time to disease progression ( TTP ) was 251 days and 252 days for anastrozole and tamoxifen , respectively .
	manualset3
176839	3	410948	13	NULL	NULL	0	NULL	252 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The median time to disease progression ( TTP ) was 251 days and 252 days for anastrozole and tamoxifen , respectively .
	manualset3
176840	4	410948	13	NULL	NULL	0	NULL	anastrozole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The median time to disease progression ( TTP ) was 251 days and 252 days for anastrozole and tamoxifen , respectively .
	manualset3
176841	5	410948	13	NULL	NULL	0	NULL	tamoxifen 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The median time to disease progression ( TTP ) was 251 days and 252 days for anastrozole and tamoxifen , respectively .
	manualset3
176842	1	410949	13	NULL	NULL	0	NULL	medical council	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The medical council on alcoholism .
	manualset3
176843	2	410949	13	NULL	NULL	0	NULL	alcoholism 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The medical council on alcoholism .
	manualset3
176844	1	410950	13	NULL	NULL	0	NULL	 tube fed O ( 2 ) gas 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A tube fed O ( 2 ) gas to the reactor chambers .
	manualset3
176845	2	410950	13	NULL	NULL	0	NULL	reactor chambers	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	A tube fed O ( 2 ) gas to the reactor chambers .
	manualset3
176846	1	410951	13	NULL	NULL	0	NULL	members	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The members of a recently identified protein family termed regulators of G-protein signaling ( RGS ) act as GTPase-activating proteins for certain Galpha subunits in vitro , but their physiological effects in cells are uncertain in the face of similar biochemical activity and overlapping patterns of tissue expression .
	manualset3
176847	2	410951	13	NULL	NULL	0	NULL	protein family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The members of a recently identified protein family termed regulators of G-protein signaling ( RGS ) act as GTPase-activating proteins for certain Galpha subunits in vitro , but their physiological effects in cells are uncertain in the face of similar biochemical activity and overlapping patterns of tissue expression .
	manualset3
176848	3	410951	13	NULL	NULL	0	NULL	regulators of G-protein signaling ( RGS ) 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The members of a recently identified protein family termed regulators of G-protein signaling ( RGS ) act as GTPase-activating proteins for certain Galpha subunits in vitro , but their physiological effects in cells are uncertain in the face of similar biochemical activity and overlapping patterns of tissue expression .
	manualset3
176850	5	410951	13	NULL	NULL	0	NULL	GTPase-activating proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The members of a recently identified protein family termed regulators of G-protein signaling ( RGS ) act as GTPase-activating proteins for certain Galpha subunits in vitro , but their physiological effects in cells are uncertain in the face of similar biochemical activity and overlapping patterns of tissue expression .
	manualset3
176851	6	410951	13	NULL	NULL	0	NULL	Galpha subunits	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The members of a recently identified protein family termed regulators of G-protein signaling ( RGS ) act as GTPase-activating proteins for certain Galpha subunits in vitro , but their physiological effects in cells are uncertain in the face of similar biochemical activity and overlapping patterns of tissue expression .
	manualset3
176852	7	410951	13	NULL	NULL	0	NULL	physiological effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The members of a recently identified protein family termed regulators of G-protein signaling ( RGS ) act as GTPase-activating proteins for certain Galpha subunits in vitro , but their physiological effects in cells are uncertain in the face of similar biochemical activity and overlapping patterns of tissue expression .
	manualset3
176853	8	410951	13	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The members of a recently identified protein family termed regulators of G-protein signaling ( RGS ) act as GTPase-activating proteins for certain Galpha subunits in vitro , but their physiological effects in cells are uncertain in the face of similar biochemical activity and overlapping patterns of tissue expression .
	manualset3
176854	9	410951	13	NULL	NULL	0	NULL	biochemical activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The members of a recently identified protein family termed regulators of G-protein signaling ( RGS ) act as GTPase-activating proteins for certain Galpha subunits in vitro , but their physiological effects in cells are uncertain in the face of similar biochemical activity and overlapping patterns of tissue expression .
	manualset3
176855	10	410951	13	NULL	NULL	0	NULL	overlapping patterns 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The members of a recently identified protein family termed regulators of G-protein signaling ( RGS ) act as GTPase-activating proteins for certain Galpha subunits in vitro , but their physiological effects in cells are uncertain in the face of similar biochemical activity and overlapping patterns of tissue expression .
	manualset3
176856	11	410951	13	NULL	NULL	0	NULL	tissue expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The members of a recently identified protein family termed regulators of G-protein signaling ( RGS ) act as GTPase-activating proteins for certain Galpha subunits in vitro , but their physiological effects in cells are uncertain in the face of similar biochemical activity and overlapping patterns of tissue expression .
	manualset3
176857	1	410952	13	NULL	NULL	0	NULL	membrane 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The membrane potential varied between -8 and -90 mV .
	manualset3
176858	2	410952	13	NULL	NULL	0	NULL	-8 and -90 mV	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The membrane potential varied between -8 and -90 mV .
	manualset3
176859	1	410953	13	NULL	NULL	0	NULL	meshwork	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The meshwork was positive with PA-TCH-SP , DI , and HID .
	manualset3
176860	2	410953	13	NULL	NULL	0	NULL	PA-TCH-SP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The meshwork was positive with PA-TCH-SP , DI , and HID .
	manualset3
176861	3	410953	13	NULL	NULL	0	NULL	DI	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The meshwork was positive with PA-TCH-SP , DI , and HID .
	manualset3
176862	4	410953	13	NULL	NULL	0	NULL	HID	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The meshwork was positive with PA-TCH-SP , DI , and HID .
	manualset3
176863	1	410954	13	NULL	NULL	0	NULL	message 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The message for this transcription factor is up-regulated by P. indica .
	manualset3
176864	2	410954	13	NULL	NULL	0	NULL	 transcription factor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The message for this transcription factor is up-regulated by P. indica .
	manualset3
176865	3	410954	13	NULL	NULL	0	NULL	P. indica	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The message for this transcription factor is up-regulated by P. indica .
	manualset3
176866	1	410955	13	NULL	NULL	0	NULL	messenger RNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The messenger RNAs for the outer membrane proteins in E. coli are more stable than the bulk of the messenger RNA s ( Hirashima et al. , 1973 ) .
	manualset3
176867	2	410955	13	NULL	NULL	0	NULL	outer membrane proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The messenger RNAs for the outer membrane proteins in E. coli are more stable than the bulk of the messenger RNA s ( Hirashima et al. , 1973 ) .
	manualset3
176868	3	410955	13	NULL	NULL	0	NULL	E. coli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The messenger RNAs for the outer membrane proteins in E. coli are more stable than the bulk of the messenger RNA s ( Hirashima et al. , 1973 ) .
	manualset3
176869	4	410955	13	NULL	NULL	0	NULL	bulk 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The messenger RNAs for the outer membrane proteins in E. coli are more stable than the bulk of the messenger RNA s ( Hirashima et al. , 1973 ) .
	manualset3
176870	5	410955	13	NULL	NULL	0	NULL	messenger RNA s 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The messenger RNAs for the outer membrane proteins in E. coli are more stable than the bulk of the messenger RNA s ( Hirashima et al. , 1973 ) .
	manualset3
176871	6	410955	13	NULL	NULL	0	NULL	Hirashima et al.	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The messenger RNAs for the outer membrane proteins in E. coli are more stable than the bulk of the messenger RNA s ( Hirashima et al. , 1973 ) .
	manualset3
176872	7	410955	13	NULL	NULL	0	NULL	1973	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The messenger RNAs for the outer membrane proteins in E. coli are more stable than the bulk of the messenger RNA s ( Hirashima et al. , 1973 ) .
	manualset3
176873	1	410956	13	NULL	NULL	0	NULL	metabolic changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic and perfusional changes in the cerebral cortex of ALS patients are likely to depend on upper motor neuron involvement , but they are not confined to the neurons of the corticospinal tract .
	manualset3
176874	2	410956	13	NULL	NULL	0	NULL	perfusional changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic and perfusional changes in the cerebral cortex of ALS patients are likely to depend on upper motor neuron involvement , but they are not confined to the neurons of the corticospinal tract .
	manualset3
176875	3	410956	13	NULL	NULL	0	NULL	cerebral cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic and perfusional changes in the cerebral cortex of ALS patients are likely to depend on upper motor neuron involvement , but they are not confined to the neurons of the corticospinal tract .
	manualset3
176876	4	410956	13	NULL	NULL	0	NULL	ALS patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic and perfusional changes in the cerebral cortex of ALS patients are likely to depend on upper motor neuron involvement , but they are not confined to the neurons of the corticospinal tract .
	manualset3
176877	5	410956	13	NULL	NULL	0	NULL	motor neuron	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic and perfusional changes in the cerebral cortex of ALS patients are likely to depend on upper motor neuron involvement , but they are not confined to the neurons of the corticospinal tract .
	manualset3
176878	6	410956	13	NULL	NULL	0	NULL	involvement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic and perfusional changes in the cerebral cortex of ALS patients are likely to depend on upper motor neuron involvement , but they are not confined to the neurons of the corticospinal tract .
	manualset3
176879	7	410956	13	NULL	NULL	0	NULL	neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic and perfusional changes in the cerebral cortex of ALS patients are likely to depend on upper motor neuron involvement , but they are not confined to the neurons of the corticospinal tract .
	manualset3
176880	8	410956	13	NULL	NULL	0	NULL	corticospinal tract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic and perfusional changes in the cerebral cortex of ALS patients are likely to depend on upper motor neuron involvement , but they are not confined to the neurons of the corticospinal tract .
	manualset3
176881	1	410957	13	NULL	NULL	0	NULL	metabolic changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic changes include the elevation of urinary alpha-hydroxy-n-valerate , o - and p-HPA , PAG , nicotinate and hippurate accompanied by decreases in the levels of urinary alpha-ketoglutarate , succinate , citrate , N-methylnicotinamide , NAG , DMA , allantoin and acetate following USPIO administration .
	manualset3
176882	2	410957	13	NULL	NULL	0	NULL	elevation	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic changes include the elevation of urinary alpha-hydroxy-n-valerate , o - and p-HPA , PAG , nicotinate and hippurate accompanied by decreases in the levels of urinary alpha-ketoglutarate , succinate , citrate , N-methylnicotinamide , NAG , DMA , allantoin and acetate following USPIO administration .
	manualset3
176883	3	410957	13	NULL	NULL	0	NULL	urinary alpha-hydroxy-n-valerate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic changes include the elevation of urinary alpha-hydroxy-n-valerate , o - and p-HPA , PAG , nicotinate and hippurate accompanied by decreases in the levels of urinary alpha-ketoglutarate , succinate , citrate , N-methylnicotinamide , NAG , DMA , allantoin and acetate following USPIO administration .
	manualset3
176884	4	410957	13	NULL	NULL	0	NULL	o - and p-HPA 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic changes include the elevation of urinary alpha-hydroxy-n-valerate , o - and p-HPA , PAG , nicotinate and hippurate accompanied by decreases in the levels of urinary alpha-ketoglutarate , succinate , citrate , N-methylnicotinamide , NAG , DMA , allantoin and acetate following USPIO administration .
	manualset3
176885	5	410957	13	NULL	NULL	0	NULL	PAG	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic changes include the elevation of urinary alpha-hydroxy-n-valerate , o - and p-HPA , PAG , nicotinate and hippurate accompanied by decreases in the levels of urinary alpha-ketoglutarate , succinate , citrate , N-methylnicotinamide , NAG , DMA , allantoin and acetate following USPIO administration .
	manualset3
176886	6	410957	13	NULL	NULL	0	NULL	nicotinate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic changes include the elevation of urinary alpha-hydroxy-n-valerate , o - and p-HPA , PAG , nicotinate and hippurate accompanied by decreases in the levels of urinary alpha-ketoglutarate , succinate , citrate , N-methylnicotinamide , NAG , DMA , allantoin and acetate following USPIO administration .
	manualset3
176887	7	410957	13	NULL	NULL	0	NULL	hippurate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic changes include the elevation of urinary alpha-hydroxy-n-valerate , o - and p-HPA , PAG , nicotinate and hippurate accompanied by decreases in the levels of urinary alpha-ketoglutarate , succinate , citrate , N-methylnicotinamide , NAG , DMA , allantoin and acetate following USPIO administration .
	manualset3
176888	8	410957	13	NULL	NULL	0	NULL	 levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic changes include the elevation of urinary alpha-hydroxy-n-valerate , o - and p-HPA , PAG , nicotinate and hippurate accompanied by decreases in the levels of urinary alpha-ketoglutarate , succinate , citrate , N-methylnicotinamide , NAG , DMA , allantoin and acetate following USPIO administration .
	manualset3
176889	9	410957	13	NULL	NULL	0	NULL	urinary alpha-ketoglutarate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic changes include the elevation of urinary alpha-hydroxy-n-valerate , o - and p-HPA , PAG , nicotinate and hippurate accompanied by decreases in the levels of urinary alpha-ketoglutarate , succinate , citrate , N-methylnicotinamide , NAG , DMA , allantoin and acetate following USPIO administration .
	manualset3
176890	10	410957	13	NULL	NULL	0	NULL	succinate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic changes include the elevation of urinary alpha-hydroxy-n-valerate , o - and p-HPA , PAG , nicotinate and hippurate accompanied by decreases in the levels of urinary alpha-ketoglutarate , succinate , citrate , N-methylnicotinamide , NAG , DMA , allantoin and acetate following USPIO administration .
	manualset3
176891	11	410957	13	NULL	NULL	0	NULL	 citrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic changes include the elevation of urinary alpha-hydroxy-n-valerate , o - and p-HPA , PAG , nicotinate and hippurate accompanied by decreases in the levels of urinary alpha-ketoglutarate , succinate , citrate , N-methylnicotinamide , NAG , DMA , allantoin and acetate following USPIO administration .
	manualset3
176892	12	410957	13	NULL	NULL	0	NULL	N-methylnicotinamide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic changes include the elevation of urinary alpha-hydroxy-n-valerate , o - and p-HPA , PAG , nicotinate and hippurate accompanied by decreases in the levels of urinary alpha-ketoglutarate , succinate , citrate , N-methylnicotinamide , NAG , DMA , allantoin and acetate following USPIO administration .
	manualset3
176893	13	410957	13	NULL	NULL	0	NULL	 NAG	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic changes include the elevation of urinary alpha-hydroxy-n-valerate , o - and p-HPA , PAG , nicotinate and hippurate accompanied by decreases in the levels of urinary alpha-ketoglutarate , succinate , citrate , N-methylnicotinamide , NAG , DMA , allantoin and acetate following USPIO administration .
	manualset3
176894	14	410957	13	NULL	NULL	0	NULL	DMA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic changes include the elevation of urinary alpha-hydroxy-n-valerate , o - and p-HPA , PAG , nicotinate and hippurate accompanied by decreases in the levels of urinary alpha-ketoglutarate , succinate , citrate , N-methylnicotinamide , NAG , DMA , allantoin and acetate following USPIO administration .
	manualset3
176895	15	410957	13	NULL	NULL	0	NULL	allantoin 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic changes include the elevation of urinary alpha-hydroxy-n-valerate , o - and p-HPA , PAG , nicotinate and hippurate accompanied by decreases in the levels of urinary alpha-ketoglutarate , succinate , citrate , N-methylnicotinamide , NAG , DMA , allantoin and acetate following USPIO administration .
	manualset3
176896	16	410957	13	NULL	NULL	0	NULL	acetate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic changes include the elevation of urinary alpha-hydroxy-n-valerate , o - and p-HPA , PAG , nicotinate and hippurate accompanied by decreases in the levels of urinary alpha-ketoglutarate , succinate , citrate , N-methylnicotinamide , NAG , DMA , allantoin and acetate following USPIO administration .
	manualset3
176897	17	410957	13	NULL	NULL	0	NULL	USPIO administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic changes include the elevation of urinary alpha-hydroxy-n-valerate , o - and p-HPA , PAG , nicotinate and hippurate accompanied by decreases in the levels of urinary alpha-ketoglutarate , succinate , citrate , N-methylnicotinamide , NAG , DMA , allantoin and acetate following USPIO administration .
	manualset3
176898	1	410958	13	NULL	NULL	0	NULL	tuberculosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A tuberculosis caused by resistant or even multidrug-resistant TB bacilli seems to be of increasing importance in some parts of the world .
	manualset3
176899	2	410958	13	NULL	NULL	0	NULL	resistant or even multidrug-resistant TB bacilli 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A tuberculosis caused by resistant or even multidrug-resistant TB bacilli seems to be of increasing importance in some parts of the world .
	manualset3
176900	3	410958	13	NULL	NULL	0	NULL	importance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A tuberculosis caused by resistant or even multidrug-resistant TB bacilli seems to be of increasing importance in some parts of the world .
	manualset3
176901	4	410958	13	NULL	NULL	0	NULL	some parts of the world 	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A tuberculosis caused by resistant or even multidrug-resistant TB bacilli seems to be of increasing importance in some parts of the world .
	manualset3
176902	1	410959	13	NULL	NULL	0	NULL	metabolic clearance rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic clearance rate for five subjects was 799 + / - 89 liters/24 hr ( 470 + / - 47 liters/24 hr/sq m ) before and 751 + / - 93 liters/24 hr ( 444 + / - 57 liters/24 hr/sq m ) during therapy .
	manualset3
176903	2	410959	13	NULL	NULL	0	NULL	five subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic clearance rate for five subjects was 799 + / - 89 liters/24 hr ( 470 + / - 47 liters/24 hr/sq m ) before and 751 + / - 93 liters/24 hr ( 444 + / - 57 liters/24 hr/sq m ) during therapy .
	manualset3
176904	3	410959	13	NULL	NULL	0	NULL	799 + / - 89 liters/24 hr	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic clearance rate for five subjects was 799 + / - 89 liters/24 hr ( 470 + / - 47 liters/24 hr/sq m ) before and 751 + / - 93 liters/24 hr ( 444 + / - 57 liters/24 hr/sq m ) during therapy .
	manualset3
176905	4	410959	13	NULL	NULL	0	NULL	470 + / - 47 liters/24 hr/sq m	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic clearance rate for five subjects was 799 + / - 89 liters/24 hr ( 470 + / - 47 liters/24 hr/sq m ) before and 751 + / - 93 liters/24 hr ( 444 + / - 57 liters/24 hr/sq m ) during therapy .
	manualset3
176906	5	410959	13	NULL	NULL	0	NULL	751 + / - 93 liters/24 hr	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic clearance rate for five subjects was 799 + / - 89 liters/24 hr ( 470 + / - 47 liters/24 hr/sq m ) before and 751 + / - 93 liters/24 hr ( 444 + / - 57 liters/24 hr/sq m ) during therapy .
	manualset3
176907	6	410959	13	NULL	NULL	0	NULL	444 + / - 57 liters/24 hr/sq m	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic clearance rate for five subjects was 799 + / - 89 liters/24 hr ( 470 + / - 47 liters/24 hr/sq m ) before and 751 + / - 93 liters/24 hr ( 444 + / - 57 liters/24 hr/sq m ) during therapy .
	manualset3
176908	7	410959	13	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolic clearance rate for five subjects was 799 + / - 89 liters/24 hr ( 470 + / - 47 liters/24 hr/sq m ) before and 751 + / - 93 liters/24 hr ( 444 + / - 57 liters/24 hr/sq m ) during therapy .
	manualset3
176909	1	410960	13	NULL	NULL	0	NULL	metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolism and genotoxicity of 1 , 2-dibromoethane ( EDB ) and its deuterium substituted analog ( d4EDB ) were studied in isolated rat hepatocytes .
	manualset3
176910	2	410960	13	NULL	NULL	NULL	NULL	1 , 2-dibromoethane ( EDB )	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The metabolism and genotoxicity of 1 , 2-dibromoethane ( EDB ) and its deuterium substituted analog ( d4EDB ) were studied in isolated rat hepatocytes .
	manualset3
176911	3	410960	13	NULL	NULL	0	NULL	deuterium substituted analog ( d4EDB )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolism and genotoxicity of 1 , 2-dibromoethane ( EDB ) and its deuterium substituted analog ( d4EDB ) were studied in isolated rat hepatocytes .
	manualset3
176912	4	410960	13	NULL	NULL	0	NULL	isolated rat hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolism and genotoxicity of 1 , 2-dibromoethane ( EDB ) and its deuterium substituted analog ( d4EDB ) were studied in isolated rat hepatocytes .
	manualset3
176913	5	410960	13	NULL	NULL	0	NULL	 genotoxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolism and genotoxicity of 1 , 2-dibromoethane ( EDB ) and its deuterium substituted analog ( d4EDB ) were studied in isolated rat hepatocytes .
	manualset3
176914	1	410961	13	NULL	NULL	0	NULL	metabolism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolism of Odapipam has been studied with phenobarbital-induced rat liver microsomes , followed by analysis with normal-phase hplc in combination with particle-beam mass spectrometry .
	manualset3
176915	2	410961	13	NULL	NULL	0	NULL	Odapipam	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolism of Odapipam has been studied with phenobarbital-induced rat liver microsomes , followed by analysis with normal-phase hplc in combination with particle-beam mass spectrometry .
	manualset3
176916	3	410961	13	NULL	NULL	0	NULL	rat liver microsomes 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolism of Odapipam has been studied with phenobarbital-induced rat liver microsomes , followed by analysis with normal-phase hplc in combination with particle-beam mass spectrometry .
	manualset3
176917	4	410961	13	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolism of Odapipam has been studied with phenobarbital-induced rat liver microsomes , followed by analysis with normal-phase hplc in combination with particle-beam mass spectrometry .
	manualset3
176918	5	410961	13	NULL	NULL	0	NULL	normal-phase hplc 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolism of Odapipam has been studied with phenobarbital-induced rat liver microsomes , followed by analysis with normal-phase hplc in combination with particle-beam mass spectrometry .
	manualset3
176919	6	410961	13	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolism of Odapipam has been studied with phenobarbital-induced rat liver microsomes , followed by analysis with normal-phase hplc in combination with particle-beam mass spectrometry .
	manualset3
176920	7	410961	13	NULL	NULL	0	NULL	particle-beam mass spectrometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolism of Odapipam has been studied with phenobarbital-induced rat liver microsomes , followed by analysis with normal-phase hplc in combination with particle-beam mass spectrometry .
	manualset3
176921	1	410962	13	NULL	NULL	0	NULL	metabolism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolism of pteroylglutamic acid by the rat .
	manualset3
176922	2	410962	13	NULL	NULL	0	NULL	pteroylglutamic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolism of pteroylglutamic acid by the rat .
	manualset3
176923	3	410962	13	NULL	NULL	0	NULL	rat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolism of pteroylglutamic acid by the rat .
	manualset3
176924	1	410963	13	NULL	NULL	0	NULL	metacarpal index ( MCI )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The metacarpal index ( MCI ) , sigma gray scale/diameter ( sigma GS/D ) and bone mineral content ( BMC ) were measured as bone mass indices , and the relationship investigated between clinical factors ( age , duration of hemodialysis , serum phosphate ( P ) , calcium ( Ca ) , carboxy-terminal fragments of parathyroid hormone ( C-PTH ) , osteocalcin ( OC ) , alkaline phosphate ( ALP ) and Ca x P ) .
	manualset3
176925	2	410963	13	NULL	NULL	0	NULL	sigma gray scale/diameter ( sigma GS/D )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The metacarpal index ( MCI ) , sigma gray scale/diameter ( sigma GS/D ) and bone mineral content ( BMC ) were measured as bone mass indices , and the relationship investigated between clinical factors ( age , duration of hemodialysis , serum phosphate ( P ) , calcium ( Ca ) , carboxy-terminal fragments of parathyroid hormone ( C-PTH ) , osteocalcin ( OC ) , alkaline phosphate ( ALP ) and Ca x P ) .
	manualset3
176926	3	410963	13	NULL	NULL	0	NULL	 bone mineral content ( BMC ) 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The metacarpal index ( MCI ) , sigma gray scale/diameter ( sigma GS/D ) and bone mineral content ( BMC ) were measured as bone mass indices , and the relationship investigated between clinical factors ( age , duration of hemodialysis , serum phosphate ( P ) , calcium ( Ca ) , carboxy-terminal fragments of parathyroid hormone ( C-PTH ) , osteocalcin ( OC ) , alkaline phosphate ( ALP ) and Ca x P ) .
	manualset3
176927	4	410963	13	NULL	NULL	0	NULL	bone mass indices	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The metacarpal index ( MCI ) , sigma gray scale/diameter ( sigma GS/D ) and bone mineral content ( BMC ) were measured as bone mass indices , and the relationship investigated between clinical factors ( age , duration of hemodialysis , serum phosphate ( P ) , calcium ( Ca ) , carboxy-terminal fragments of parathyroid hormone ( C-PTH ) , osteocalcin ( OC ) , alkaline phosphate ( ALP ) and Ca x P ) .
	manualset3
176928	5	410963	13	NULL	NULL	0	NULL	relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The metacarpal index ( MCI ) , sigma gray scale/diameter ( sigma GS/D ) and bone mineral content ( BMC ) were measured as bone mass indices , and the relationship investigated between clinical factors ( age , duration of hemodialysis , serum phosphate ( P ) , calcium ( Ca ) , carboxy-terminal fragments of parathyroid hormone ( C-PTH ) , osteocalcin ( OC ) , alkaline phosphate ( ALP ) and Ca x P ) .
	manualset3
176929	6	410963	13	NULL	NULL	0	NULL	clinical factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The metacarpal index ( MCI ) , sigma gray scale/diameter ( sigma GS/D ) and bone mineral content ( BMC ) were measured as bone mass indices , and the relationship investigated between clinical factors ( age , duration of hemodialysis , serum phosphate ( P ) , calcium ( Ca ) , carboxy-terminal fragments of parathyroid hormone ( C-PTH ) , osteocalcin ( OC ) , alkaline phosphate ( ALP ) and Ca x P ) .
	manualset3
176930	7	410963	13	NULL	NULL	0	NULL	age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The metacarpal index ( MCI ) , sigma gray scale/diameter ( sigma GS/D ) and bone mineral content ( BMC ) were measured as bone mass indices , and the relationship investigated between clinical factors ( age , duration of hemodialysis , serum phosphate ( P ) , calcium ( Ca ) , carboxy-terminal fragments of parathyroid hormone ( C-PTH ) , osteocalcin ( OC ) , alkaline phosphate ( ALP ) and Ca x P ) .
	manualset3
176931	8	410963	13	NULL	NULL	0	NULL	duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The metacarpal index ( MCI ) , sigma gray scale/diameter ( sigma GS/D ) and bone mineral content ( BMC ) were measured as bone mass indices , and the relationship investigated between clinical factors ( age , duration of hemodialysis , serum phosphate ( P ) , calcium ( Ca ) , carboxy-terminal fragments of parathyroid hormone ( C-PTH ) , osteocalcin ( OC ) , alkaline phosphate ( ALP ) and Ca x P ) .
	manualset3
176932	9	410963	13	NULL	NULL	0	NULL	hemodialysis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The metacarpal index ( MCI ) , sigma gray scale/diameter ( sigma GS/D ) and bone mineral content ( BMC ) were measured as bone mass indices , and the relationship investigated between clinical factors ( age , duration of hemodialysis , serum phosphate ( P ) , calcium ( Ca ) , carboxy-terminal fragments of parathyroid hormone ( C-PTH ) , osteocalcin ( OC ) , alkaline phosphate ( ALP ) and Ca x P ) .
	manualset3
176933	10	410963	13	NULL	NULL	0	NULL	serum phosphate ( P ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The metacarpal index ( MCI ) , sigma gray scale/diameter ( sigma GS/D ) and bone mineral content ( BMC ) were measured as bone mass indices , and the relationship investigated between clinical factors ( age , duration of hemodialysis , serum phosphate ( P ) , calcium ( Ca ) , carboxy-terminal fragments of parathyroid hormone ( C-PTH ) , osteocalcin ( OC ) , alkaline phosphate ( ALP ) and Ca x P ) .
	manualset3
176934	11	410963	13	NULL	NULL	0	NULL	calcium ( Ca ) 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The metacarpal index ( MCI ) , sigma gray scale/diameter ( sigma GS/D ) and bone mineral content ( BMC ) were measured as bone mass indices , and the relationship investigated between clinical factors ( age , duration of hemodialysis , serum phosphate ( P ) , calcium ( Ca ) , carboxy-terminal fragments of parathyroid hormone ( C-PTH ) , osteocalcin ( OC ) , alkaline phosphate ( ALP ) and Ca x P ) .
	manualset3
176935	12	410963	13	NULL	NULL	0	NULL	carboxy-terminal fragments 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The metacarpal index ( MCI ) , sigma gray scale/diameter ( sigma GS/D ) and bone mineral content ( BMC ) were measured as bone mass indices , and the relationship investigated between clinical factors ( age , duration of hemodialysis , serum phosphate ( P ) , calcium ( Ca ) , carboxy-terminal fragments of parathyroid hormone ( C-PTH ) , osteocalcin ( OC ) , alkaline phosphate ( ALP ) and Ca x P ) .
	manualset3
176936	13	410963	13	NULL	NULL	0	NULL	parathyroid hormone ( C-PTH )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The metacarpal index ( MCI ) , sigma gray scale/diameter ( sigma GS/D ) and bone mineral content ( BMC ) were measured as bone mass indices , and the relationship investigated between clinical factors ( age , duration of hemodialysis , serum phosphate ( P ) , calcium ( Ca ) , carboxy-terminal fragments of parathyroid hormone ( C-PTH ) , osteocalcin ( OC ) , alkaline phosphate ( ALP ) and Ca x P ) .
	manualset3
176937	14	410963	13	NULL	NULL	0	NULL	osteocalcin ( OC ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The metacarpal index ( MCI ) , sigma gray scale/diameter ( sigma GS/D ) and bone mineral content ( BMC ) were measured as bone mass indices , and the relationship investigated between clinical factors ( age , duration of hemodialysis , serum phosphate ( P ) , calcium ( Ca ) , carboxy-terminal fragments of parathyroid hormone ( C-PTH ) , osteocalcin ( OC ) , alkaline phosphate ( ALP ) and Ca x P ) .
	manualset3
176938	15	410963	13	NULL	NULL	0	NULL	alkaline phosphate ( ALP )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The metacarpal index ( MCI ) , sigma gray scale/diameter ( sigma GS/D ) and bone mineral content ( BMC ) were measured as bone mass indices , and the relationship investigated between clinical factors ( age , duration of hemodialysis , serum phosphate ( P ) , calcium ( Ca ) , carboxy-terminal fragments of parathyroid hormone ( C-PTH ) , osteocalcin ( OC ) , alkaline phosphate ( ALP ) and Ca x P ) .
	manualset3
176939	16	410963	13	NULL	NULL	0	NULL	 Ca x P	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The metacarpal index ( MCI ) , sigma gray scale/diameter ( sigma GS/D ) and bone mineral content ( BMC ) were measured as bone mass indices , and the relationship investigated between clinical factors ( age , duration of hemodialysis , serum phosphate ( P ) , calcium ( Ca ) , carboxy-terminal fragments of parathyroid hormone ( C-PTH ) , osteocalcin ( OC ) , alkaline phosphate ( ALP ) and Ca x P ) .
	manualset3
176940	1	410964	13	NULL	NULL	0	NULL	metal sites	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The metal sites on sarcoplasmic reticulum membranes that bind lanthanide ions with the highest affinity are not the ATPase Ca2 + transport sites .
	manualset3
176941	2	410964	13	NULL	NULL	0	NULL	sarcoplasmic reticulum membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The metal sites on sarcoplasmic reticulum membranes that bind lanthanide ions with the highest affinity are not the ATPase Ca2 + transport sites .
	manualset3
176943	4	410964	13	NULL	NULL	0	NULL	lanthanide ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The metal sites on sarcoplasmic reticulum membranes that bind lanthanide ions with the highest affinity are not the ATPase Ca2 + transport sites .
	manualset3
176944	5	410964	13	NULL	NULL	0	NULL	highest affinity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The metal sites on sarcoplasmic reticulum membranes that bind lanthanide ions with the highest affinity are not the ATPase Ca2 + transport sites .
	manualset3
176945	6	410964	13	NULL	NULL	0	NULL	ATPase Ca2 + transport sites	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The metal sites on sarcoplasmic reticulum membranes that bind lanthanide ions with the highest affinity are not the ATPase Ca2 + transport sites .
	manualset3
176946	1	410965	13	NULL	NULL	0	NULL	metals 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The metals are placed in either the phosphorus/thioether or the phosphorus/ether coordination pocket of the dissymmetric ligand by taking advantage of the stepwise synthetic control offered by the weak-link approach .
	manualset3
176947	2	410965	13	NULL	NULL	0	NULL	 phosphorus/thioether	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The metals are placed in either the phosphorus/thioether or the phosphorus/ether coordination pocket of the dissymmetric ligand by taking advantage of the stepwise synthetic control offered by the weak-link approach .
	manualset3
176948	3	410965	13	NULL	NULL	0	NULL	phosphorus/ether	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The metals are placed in either the phosphorus/thioether or the phosphorus/ether coordination pocket of the dissymmetric ligand by taking advantage of the stepwise synthetic control offered by the weak-link approach .
	manualset3
176949	4	410965	13	NULL	NULL	0	NULL	coordination pocket	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The metals are placed in either the phosphorus/thioether or the phosphorus/ether coordination pocket of the dissymmetric ligand by taking advantage of the stepwise synthetic control offered by the weak-link approach .
	manualset3
176950	5	410965	13	NULL	NULL	0	NULL	dissymmetric ligand 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The metals are placed in either the phosphorus/thioether or the phosphorus/ether coordination pocket of the dissymmetric ligand by taking advantage of the stepwise synthetic control offered by the weak-link approach .
	manualset3
176951	6	410965	13	NULL	NULL	0	NULL	advantage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The metals are placed in either the phosphorus/thioether or the phosphorus/ether coordination pocket of the dissymmetric ligand by taking advantage of the stepwise synthetic control offered by the weak-link approach .
	manualset3
176952	7	410965	13	NULL	NULL	0	NULL	stepwise synthetic control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The metals are placed in either the phosphorus/thioether or the phosphorus/ether coordination pocket of the dissymmetric ligand by taking advantage of the stepwise synthetic control offered by the weak-link approach .
	manualset3
176953	8	410965	13	NULL	NULL	0	NULL	weak-link approach	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The metals are placed in either the phosphorus/thioether or the phosphorus/ether coordination pocket of the dissymmetric ligand by taking advantage of the stepwise synthetic control offered by the weak-link approach .
	manualset3
176954	1	410966	13	NULL	NULL	0	NULL	metastability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The metastability is expected to give rise to force hysteresis in , e.g. , atomic force microscope or surface force apparatus experiments , distinctly different from those due to mechanical instabilities of the cantilever system .
	manualset3
176955	2	410966	13	NULL	NULL	0	NULL	rise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The metastability is expected to give rise to force hysteresis in , e.g. , atomic force microscope or surface force apparatus experiments , distinctly different from those due to mechanical instabilities of the cantilever system .
	manualset3
176956	3	410966	13	NULL	NULL	0	NULL	force hysteresis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The metastability is expected to give rise to force hysteresis in , e.g. , atomic force microscope or surface force apparatus experiments , distinctly different from those due to mechanical instabilities of the cantilever system .
	manualset3
176957	4	410966	13	NULL	NULL	0	NULL	atomic force microscope	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The metastability is expected to give rise to force hysteresis in , e.g. , atomic force microscope or surface force apparatus experiments , distinctly different from those due to mechanical instabilities of the cantilever system .
	manualset3
176958	5	410966	13	NULL	NULL	0	NULL	surface force apparatus experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The metastability is expected to give rise to force hysteresis in , e.g. , atomic force microscope or surface force apparatus experiments , distinctly different from those due to mechanical instabilities of the cantilever system .
	manualset3
176959	6	410966	13	NULL	NULL	0	NULL	mechanical instabilities 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The metastability is expected to give rise to force hysteresis in , e.g. , atomic force microscope or surface force apparatus experiments , distinctly different from those due to mechanical instabilities of the cantilever system .
	manualset3
176960	7	410966	13	NULL	NULL	0	NULL	cantilever system	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The metastability is expected to give rise to force hysteresis in , e.g. , atomic force microscope or surface force apparatus experiments , distinctly different from those due to mechanical instabilities of the cantilever system .
	manualset3
176961	1	410967	13	NULL	NULL	0	NULL	twin cohort study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A twin cohort study would serve a powerful tool responding to this knowledge gap by providing information on factors affecting DP when controlling for family background .
	manualset3
176962	2	410967	13	NULL	NULL	0	NULL	powerful tool	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A twin cohort study would serve a powerful tool responding to this knowledge gap by providing information on factors affecting DP when controlling for family background .
	manualset3
176963	3	410967	13	NULL	NULL	NULL	NULL	knowledge gap	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A twin cohort study would serve a powerful tool responding to this knowledge gap by providing information on factors affecting DP when controlling for family background .
	manualset3
176964	4	410967	13	NULL	NULL	0	NULL	information	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A twin cohort study would serve a powerful tool responding to this knowledge gap by providing information on factors affecting DP when controlling for family background .
	manualset3
176965	5	410967	13	NULL	NULL	0	NULL	factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A twin cohort study would serve a powerful tool responding to this knowledge gap by providing information on factors affecting DP when controlling for family background .
	manualset3
176966	6	410967	13	NULL	NULL	0	NULL	DP	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A twin cohort study would serve a powerful tool responding to this knowledge gap by providing information on factors affecting DP when controlling for family background .
	manualset3
176967	7	410967	13	NULL	NULL	0	NULL	 family background	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A twin cohort study would serve a powerful tool responding to this knowledge gap by providing information on factors affecting DP when controlling for family background .
	manualset3
176968	1	410968	13	NULL	NULL	0	NULL	method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The method , which can be combined with other water suppression schemes , is demonstrated for 2D TOCSY , NOESY , and ROESY spectra of the protein , ubiquitin in aqueous solution .
	manualset3
176969	2	410968	13	NULL	NULL	0	NULL	water suppression schemes	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The method , which can be combined with other water suppression schemes , is demonstrated for 2D TOCSY , NOESY , and ROESY spectra of the protein , ubiquitin in aqueous solution .
	manualset3
176970	3	410968	13	NULL	NULL	0	NULL	 2D TOCSY	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method , which can be combined with other water suppression schemes , is demonstrated for 2D TOCSY , NOESY , and ROESY spectra of the protein , ubiquitin in aqueous solution .
	manualset3
176971	4	410968	13	NULL	NULL	0	NULL	NOESY	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method , which can be combined with other water suppression schemes , is demonstrated for 2D TOCSY , NOESY , and ROESY spectra of the protein , ubiquitin in aqueous solution .
	manualset3
176972	5	410968	13	NULL	NULL	0	NULL	ROESY spectra	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method , which can be combined with other water suppression schemes , is demonstrated for 2D TOCSY , NOESY , and ROESY spectra of the protein , ubiquitin in aqueous solution .
	manualset3
176973	6	410968	13	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The method , which can be combined with other water suppression schemes , is demonstrated for 2D TOCSY , NOESY , and ROESY spectra of the protein , ubiquitin in aqueous solution .
	manualset3
176974	7	410968	13	NULL	NULL	0	NULL	 ubiquitin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The method , which can be combined with other water suppression schemes , is demonstrated for 2D TOCSY , NOESY , and ROESY spectra of the protein , ubiquitin in aqueous solution .
	manualset3
176975	8	410968	13	NULL	NULL	0	NULL	aqueous solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The method , which can be combined with other water suppression schemes , is demonstrated for 2D TOCSY , NOESY , and ROESY spectra of the protein , ubiquitin in aqueous solution .
	manualset3
176976	1	410969	13	NULL	NULL	0	NULL	method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The method can accommodate normal and non-normal response data and a large number of covariates .
	manualset3
176977	2	410969	13	NULL	NULL	0	NULL	normal response data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The method can accommodate normal and non-normal response data and a large number of covariates .
	manualset3
176978	3	410969	13	NULL	NULL	0	NULL	non-normal response data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The method can accommodate normal and non-normal response data and a large number of covariates .
	manualset3
176979	4	410969	13	NULL	NULL	0	NULL	number of covariates 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method can accommodate normal and non-normal response data and a large number of covariates .
	manualset3
176980	1	410970	13	NULL	NULL	0	NULL	method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method could measure plasma bromocriptine at concentrations of 0.05 nmol/L , had between-assay coefficients of variation of less than 10 % and was more convenient than previous assays using tritium radiolabels .
	manualset3
176981	2	410970	13	NULL	NULL	0	NULL	plasma bromocriptine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The method could measure plasma bromocriptine at concentrations of 0.05 nmol/L , had between-assay coefficients of variation of less than 10 % and was more convenient than previous assays using tritium radiolabels .
	manualset3
176982	3	410970	13	NULL	NULL	0	NULL	concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method could measure plasma bromocriptine at concentrations of 0.05 nmol/L , had between-assay coefficients of variation of less than 10 % and was more convenient than previous assays using tritium radiolabels .
	manualset3
176983	4	410970	13	NULL	NULL	0	NULL	0.05 nmol/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method could measure plasma bromocriptine at concentrations of 0.05 nmol/L , had between-assay coefficients of variation of less than 10 % and was more convenient than previous assays using tritium radiolabels .
	manualset3
176984	5	410970	13	NULL	NULL	0	NULL	between-assay coefficients	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method could measure plasma bromocriptine at concentrations of 0.05 nmol/L , had between-assay coefficients of variation of less than 10 % and was more convenient than previous assays using tritium radiolabels .
	manualset3
176985	6	410970	13	NULL	NULL	0	NULL	variation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method could measure plasma bromocriptine at concentrations of 0.05 nmol/L , had between-assay coefficients of variation of less than 10 % and was more convenient than previous assays using tritium radiolabels .
	manualset3
176986	7	410970	13	NULL	NULL	0	NULL	10 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method could measure plasma bromocriptine at concentrations of 0.05 nmol/L , had between-assay coefficients of variation of less than 10 % and was more convenient than previous assays using tritium radiolabels .
	manualset3
176987	8	410970	13	NULL	NULL	0	NULL	previous assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method could measure plasma bromocriptine at concentrations of 0.05 nmol/L , had between-assay coefficients of variation of less than 10 % and was more convenient than previous assays using tritium radiolabels .
	manualset3
176988	9	410970	13	NULL	NULL	0	NULL	tritium radiolabels	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The method could measure plasma bromocriptine at concentrations of 0.05 nmol/L , had between-assay coefficients of variation of less than 10 % and was more convenient than previous assays using tritium radiolabels .
	manualset3
177036	1	410971	13	NULL	NULL	0	NULL	method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method exhibited good accuracy ( 80.3-99 .8 % ) , precision ( 2.2-15 .2 % ) and lower limits that allowed quantification and confirmation at levels as low as 0.008 ng/m3 .
	manualset3
177037	2	410971	13	NULL	NULL	0	NULL	good accuracy	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method exhibited good accuracy ( 80.3-99 .8 % ) , precision ( 2.2-15 .2 % ) and lower limits that allowed quantification and confirmation at levels as low as 0.008 ng/m3 .
	manualset3
177038	3	410971	13	NULL	NULL	0	NULL	80.3-99 .8 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method exhibited good accuracy ( 80.3-99 .8 % ) , precision ( 2.2-15 .2 % ) and lower limits that allowed quantification and confirmation at levels as low as 0.008 ng/m3 .
	manualset3
177039	4	410971	13	NULL	NULL	0	NULL	precision	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method exhibited good accuracy ( 80.3-99 .8 % ) , precision ( 2.2-15 .2 % ) and lower limits that allowed quantification and confirmation at levels as low as 0.008 ng/m3 .
	manualset3
177040	5	410971	13	NULL	NULL	0	NULL	2.2-15 .2 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method exhibited good accuracy ( 80.3-99 .8 % ) , precision ( 2.2-15 .2 % ) and lower limits that allowed quantification and confirmation at levels as low as 0.008 ng/m3 .
	manualset3
177041	6	410971	13	NULL	NULL	0	NULL	limits	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method exhibited good accuracy ( 80.3-99 .8 % ) , precision ( 2.2-15 .2 % ) and lower limits that allowed quantification and confirmation at levels as low as 0.008 ng/m3 .
	manualset3
177042	7	410971	13	NULL	NULL	0	NULL	quantification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method exhibited good accuracy ( 80.3-99 .8 % ) , precision ( 2.2-15 .2 % ) and lower limits that allowed quantification and confirmation at levels as low as 0.008 ng/m3 .
	manualset3
177043	8	410971	13	NULL	NULL	0	NULL	confirmation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method exhibited good accuracy ( 80.3-99 .8 % ) , precision ( 2.2-15 .2 % ) and lower limits that allowed quantification and confirmation at levels as low as 0.008 ng/m3 .
	manualset3
177044	9	410971	13	NULL	NULL	0	NULL	levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method exhibited good accuracy ( 80.3-99 .8 % ) , precision ( 2.2-15 .2 % ) and lower limits that allowed quantification and confirmation at levels as low as 0.008 ng/m3 .
	manualset3
177045	10	410971	13	NULL	NULL	0	NULL	0.008 ng/m3	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method exhibited good accuracy ( 80.3-99 .8 % ) , precision ( 2.2-15 .2 % ) and lower limits that allowed quantification and confirmation at levels as low as 0.008 ng/m3 .
	manualset3
177046	1	410972	13	NULL	NULL	0	NULL	method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method has been shown to be robust and valid over a concentration range of 10-5000 ng/ml using a 0.2-ml sample volume .
	manualset3
177047	2	410972	13	NULL	NULL	0	NULL	concentration range 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method has been shown to be robust and valid over a concentration range of 10-5000 ng/ml using a 0.2-ml sample volume .
	manualset3
177048	3	410972	13	NULL	NULL	0	NULL	10-5000 ng/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method has been shown to be robust and valid over a concentration range of 10-5000 ng/ml using a 0.2-ml sample volume .
	manualset3
177049	4	410972	13	NULL	NULL	0	NULL	0.2-ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method has been shown to be robust and valid over a concentration range of 10-5000 ng/ml using a 0.2-ml sample volume .
	manualset3
177050	5	410972	13	NULL	NULL	0	NULL	sample volume	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method has been shown to be robust and valid over a concentration range of 10-5000 ng/ml using a 0.2-ml sample volume .
	manualset3
177053	1	410973	13	NULL	NULL	NULL	NULL	two-phase solvent system	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A two-phase solvent system consisting of chloroform-methanol-isopropanol-water ( 3 : 2 : 2 : 3 , v/v ) was used for HSCCC .
	manualset3
177054	2	410973	13	NULL	NULL	0	NULL	chloroform-methanol-isopropanol-water 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A two-phase solvent system consisting of chloroform-methanol-isopropanol-water ( 3 : 2 : 2 : 3 , v/v ) was used for HSCCC .
	manualset3
177055	3	410973	13	NULL	NULL	0	NULL	3 : 2 : 2 : 3 , v/v 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A two-phase solvent system consisting of chloroform-methanol-isopropanol-water ( 3 : 2 : 2 : 3 , v/v ) was used for HSCCC .
	manualset3
177056	4	410973	13	NULL	NULL	0	NULL	HSCCC	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A two-phase solvent system consisting of chloroform-methanol-isopropanol-water ( 3 : 2 : 2 : 3 , v/v ) was used for HSCCC .
	manualset3
177057	1	410974	13	NULL	NULL	0	NULL	method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method has promise for field screening of potential repellents before on-animal testing .
	manualset3
177058	2	410974	13	NULL	NULL	0	NULL	promise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method has promise for field screening of potential repellents before on-animal testing .
	manualset3
177059	3	410974	13	NULL	NULL	0	NULL	field screening 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method has promise for field screening of potential repellents before on-animal testing .
	manualset3
177060	4	410974	13	NULL	NULL	0	NULL	potential repellents 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method has promise for field screening of potential repellents before on-animal testing .
	manualset3
177061	5	410974	13	NULL	NULL	0	NULL	 testing 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method has promise for field screening of potential repellents before on-animal testing .
	manualset3
177062	1	410975	13	NULL	NULL	0	NULL	method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is applicable at the moment for the cyclic symmetry point groups - C ( i ) , C ( s ) , C ( n ) , and S ( n ) , and therefore it can be used also for chirality measures , which are the minimal of the S ( n ) measures .
	manualset3
177063	2	410975	13	NULL	NULL	0	NULL	moment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is applicable at the moment for the cyclic symmetry point groups - C ( i ) , C ( s ) , C ( n ) , and S ( n ) , and therefore it can be used also for chirality measures , which are the minimal of the S ( n ) measures .
	manualset3
177064	3	410975	13	NULL	NULL	0	NULL	cyclic symmetry point groups - C ( i ) , C ( s ) , C ( n ) , and S ( n )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is applicable at the moment for the cyclic symmetry point groups - C ( i ) , C ( s ) , C ( n ) , and S ( n ) , and therefore it can be used also for chirality measures , which are the minimal of the S ( n ) measures .
	manualset3
177065	4	410975	13	NULL	NULL	0	NULL	chirality measures 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is applicable at the moment for the cyclic symmetry point groups - C ( i ) , C ( s ) , C ( n ) , and S ( n ) , and therefore it can be used also for chirality measures , which are the minimal of the S ( n ) measures .
	manualset3
177066	5	410975	13	NULL	NULL	0	NULL	S ( n ) measures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is applicable at the moment for the cyclic symmetry point groups - C ( i ) , C ( s ) , C ( n ) , and S ( n ) , and therefore it can be used also for chirality measures , which are the minimal of the S ( n ) measures .
	manualset3
177067	1	410976	13	NULL	NULL	0	NULL	method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is based on the measurement of the intensely colored charge-transfer complex formed by the interaction of these drugs as n-electron donors with chloranilic acid as the pi-acceptor .
	manualset3
177068	2	410976	13	NULL	NULL	0	NULL	measurement 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is based on the measurement of the intensely colored charge-transfer complex formed by the interaction of these drugs as n-electron donors with chloranilic acid as the pi-acceptor .
	manualset3
177069	3	410976	13	NULL	NULL	0	NULL	charge-transfer complex	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is based on the measurement of the intensely colored charge-transfer complex formed by the interaction of these drugs as n-electron donors with chloranilic acid as the pi-acceptor .
	manualset3
177070	4	410976	13	NULL	NULL	0	NULL	interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is based on the measurement of the intensely colored charge-transfer complex formed by the interaction of these drugs as n-electron donors with chloranilic acid as the pi-acceptor .
	manualset3
177071	5	410976	13	NULL	NULL	0	NULL	drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is based on the measurement of the intensely colored charge-transfer complex formed by the interaction of these drugs as n-electron donors with chloranilic acid as the pi-acceptor .
	manualset3
177072	6	410976	13	NULL	NULL	0	NULL	n-electron donors	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is based on the measurement of the intensely colored charge-transfer complex formed by the interaction of these drugs as n-electron donors with chloranilic acid as the pi-acceptor .
	manualset3
177073	7	410976	13	NULL	NULL	0	NULL	chloranilic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is based on the measurement of the intensely colored charge-transfer complex formed by the interaction of these drugs as n-electron donors with chloranilic acid as the pi-acceptor .
	manualset3
177074	8	410976	13	NULL	NULL	0	NULL	pi-acceptor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is based on the measurement of the intensely colored charge-transfer complex formed by the interaction of these drugs as n-electron donors with chloranilic acid as the pi-acceptor .
	manualset3
177075	1	410977	13	NULL	NULL	0	NULL	method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is described in detail , and its indications and limitations are discussed .
	manualset3
177076	2	410977	13	NULL	NULL	0	NULL	detail 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is described in detail , and its indications and limitations are discussed .
	manualset3
177077	3	410977	13	NULL	NULL	0	NULL	indications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is described in detail , and its indications and limitations are discussed .
	manualset3
177078	4	410977	13	NULL	NULL	0	NULL	limitations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is described in detail , and its indications and limitations are discussed .
	manualset3
177079	1	410978	13	NULL	NULL	0	NULL	method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is easy to perform since both sequencing and assignment are automated .
	manualset3
177080	2	410978	13	NULL	NULL	0	NULL	assignment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is easy to perform since both sequencing and assignment are automated .
	manualset3
200341	3	410978	13	NULL	NULL	0	NULL	sequencing 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is easy to perform since both sequencing and assignment are automated .
	manualset3
177081	1	410979	13	NULL	NULL	0	NULL	method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is linear to 4 mmol/l of HDL-c and between-run and within-run CVs ranged from 1.01-2 .54 % .
	manualset3
177082	2	410979	13	NULL	NULL	0	NULL	4 mmol/l 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is linear to 4 mmol/l of HDL-c and between-run and within-run CVs ranged from 1.01-2 .54 % .
	manualset3
177083	3	410979	13	NULL	NULL	0	NULL	HDL-c	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is linear to 4 mmol/l of HDL-c and between-run and within-run CVs ranged from 1.01-2 .54 % .
	manualset3
177084	4	410979	13	NULL	NULL	0	NULL	within-run CVs	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is linear to 4 mmol/l of HDL-c and between-run and within-run CVs ranged from 1.01-2 .54 % .
	manualset3
177085	5	410979	13	NULL	NULL	0	NULL	1.01-2 .54 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is linear to 4 mmol/l of HDL-c and between-run and within-run CVs ranged from 1.01-2 .54 % .
	manualset3
177193	1	410980	13	NULL	NULL	0	NULL	 method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is most sensitive and permits the separation of lead ( II ) from binary mixtures containing commonly associated metal ions .
	manualset3
177194	2	410980	13	NULL	NULL	0	NULL	separation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is most sensitive and permits the separation of lead ( II ) from binary mixtures containing commonly associated metal ions .
	manualset3
177195	3	410980	13	NULL	NULL	0	NULL	 lead ( II )	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is most sensitive and permits the separation of lead ( II ) from binary mixtures containing commonly associated metal ions .
	manualset3
177196	4	410980	13	NULL	NULL	0	NULL	binary mixtures	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is most sensitive and permits the separation of lead ( II ) from binary mixtures containing commonly associated metal ions .
	manualset3
177197	5	410980	13	NULL	NULL	0	NULL	 metal ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is most sensitive and permits the separation of lead ( II ) from binary mixtures containing commonly associated metal ions .
	manualset3
177198	1	410981	13	NULL	NULL	0	NULL	method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is rapid and simple , and could be applied to evaluate the quality of this traditional Chinese medicine .
	manualset3
177199	2	410981	13	NULL	NULL	0	NULL	quality	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is rapid and simple , and could be applied to evaluate the quality of this traditional Chinese medicine .
	manualset3
177200	3	410981	13	NULL	NULL	0	NULL	traditional Chinese medicine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is rapid and simple , and could be applied to evaluate the quality of this traditional Chinese medicine .
	manualset3
177201	1	410982	13	NULL	NULL	0	NULL	method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is reproducible and accurate , with respect to demonstrating a relative standard deviation between 2.57 % and 3.30 % ( n = 10 , for 500 ng/mL ) and a relative error between 0.84 % and 6.54 % ( n = 10 , for 500 ng/mL ) , respectively .
	manualset3
177202	2	410982	13	NULL	NULL	0	NULL	standard deviation	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is reproducible and accurate , with respect to demonstrating a relative standard deviation between 2.57 % and 3.30 % ( n = 10 , for 500 ng/mL ) and a relative error between 0.84 % and 6.54 % ( n = 10 , for 500 ng/mL ) , respectively .
	manualset3
177203	3	410982	13	NULL	NULL	0	NULL	2.57 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is reproducible and accurate , with respect to demonstrating a relative standard deviation between 2.57 % and 3.30 % ( n = 10 , for 500 ng/mL ) and a relative error between 0.84 % and 6.54 % ( n = 10 , for 500 ng/mL ) , respectively .
	manualset3
177204	4	410982	13	NULL	NULL	0	NULL	3.30 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is reproducible and accurate , with respect to demonstrating a relative standard deviation between 2.57 % and 3.30 % ( n = 10 , for 500 ng/mL ) and a relative error between 0.84 % and 6.54 % ( n = 10 , for 500 ng/mL ) , respectively .
	manualset3
177205	5	410982	13	NULL	NULL	0	NULL	n = 10 , for 500 ng/mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is reproducible and accurate , with respect to demonstrating a relative standard deviation between 2.57 % and 3.30 % ( n = 10 , for 500 ng/mL ) and a relative error between 0.84 % and 6.54 % ( n = 10 , for 500 ng/mL ) , respectively .
	manualset3
177206	6	410982	13	NULL	NULL	0	NULL	 relative error	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is reproducible and accurate , with respect to demonstrating a relative standard deviation between 2.57 % and 3.30 % ( n = 10 , for 500 ng/mL ) and a relative error between 0.84 % and 6.54 % ( n = 10 , for 500 ng/mL ) , respectively .
	manualset3
177207	7	410982	13	NULL	NULL	0	NULL	0.84 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is reproducible and accurate , with respect to demonstrating a relative standard deviation between 2.57 % and 3.30 % ( n = 10 , for 500 ng/mL ) and a relative error between 0.84 % and 6.54 % ( n = 10 , for 500 ng/mL ) , respectively .
	manualset3
177208	8	410982	13	NULL	NULL	0	NULL	6.54 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is reproducible and accurate , with respect to demonstrating a relative standard deviation between 2.57 % and 3.30 % ( n = 10 , for 500 ng/mL ) and a relative error between 0.84 % and 6.54 % ( n = 10 , for 500 ng/mL ) , respectively .
	manualset3
177209	9	410982	13	NULL	NULL	0	NULL	 n = 10 , for 500 ng/mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is reproducible and accurate , with respect to demonstrating a relative standard deviation between 2.57 % and 3.30 % ( n = 10 , for 500 ng/mL ) and a relative error between 0.84 % and 6.54 % ( n = 10 , for 500 ng/mL ) , respectively .
	manualset3
177210	1	410983	13	NULL	NULL	0	NULL	method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is simple , rapid and rugged , and has been applied successfully to sample analysis for clinical studies .
	manualset3
177211	2	410983	13	NULL	NULL	0	NULL	 sample analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is simple , rapid and rugged , and has been applied successfully to sample analysis for clinical studies .
	manualset3
177212	3	410983	13	NULL	NULL	0	NULL	clinical studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is simple , rapid and rugged , and has been applied successfully to sample analysis for clinical studies .
	manualset3
177213	1	410984	13	NULL	NULL	0	NULL	method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method makes use of membrane fragments or vesicles containing transport proteins adsorbed onto solid-supported membrane-covered electrodes and allows the direct measurement of their activity .
	manualset3
177214	2	410984	13	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method makes use of membrane fragments or vesicles containing transport proteins adsorbed onto solid-supported membrane-covered electrodes and allows the direct measurement of their activity .
	manualset3
177215	3	410984	13	NULL	NULL	0	NULL	membrane fragments 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The method makes use of membrane fragments or vesicles containing transport proteins adsorbed onto solid-supported membrane-covered electrodes and allows the direct measurement of their activity .
	manualset3
177216	4	410984	13	NULL	NULL	NULL	NULL	vesicles	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The method makes use of membrane fragments or vesicles containing transport proteins adsorbed onto solid-supported membrane-covered electrodes and allows the direct measurement of their activity .
	manualset3
177217	5	410984	13	NULL	NULL	0	NULL	transport proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The method makes use of membrane fragments or vesicles containing transport proteins adsorbed onto solid-supported membrane-covered electrodes and allows the direct measurement of their activity .
	manualset3
177218	6	410984	13	NULL	NULL	0	NULL	 electrodes	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The method makes use of membrane fragments or vesicles containing transport proteins adsorbed onto solid-supported membrane-covered electrodes and allows the direct measurement of their activity .
	manualset3
177219	7	410984	13	NULL	NULL	0	NULL	measurement	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method makes use of membrane fragments or vesicles containing transport proteins adsorbed onto solid-supported membrane-covered electrodes and allows the direct measurement of their activity .
	manualset3
177220	8	410984	13	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The method makes use of membrane fragments or vesicles containing transport proteins adsorbed onto solid-supported membrane-covered electrodes and allows the direct measurement of their activity .
	manualset3
177221	1	410985	13	NULL	NULL	0	NULL	method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method may fail in large imaging objects such as the human trunk at high magnetic field where standing wave and RF penetration effects cause intensity variations that can not be corrected .
	manualset3
177222	2	410985	13	NULL	NULL	0	NULL	imaging objects	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The method may fail in large imaging objects such as the human trunk at high magnetic field where standing wave and RF penetration effects cause intensity variations that can not be corrected .
	manualset3
177223	3	410985	13	NULL	NULL	0	NULL	human trunk	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The method may fail in large imaging objects such as the human trunk at high magnetic field where standing wave and RF penetration effects cause intensity variations that can not be corrected .
	manualset3
177224	4	410985	13	NULL	NULL	0	NULL	magnetic field 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method may fail in large imaging objects such as the human trunk at high magnetic field where standing wave and RF penetration effects cause intensity variations that can not be corrected .
	manualset3
177225	5	410985	13	NULL	NULL	0	NULL	wave	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method may fail in large imaging objects such as the human trunk at high magnetic field where standing wave and RF penetration effects cause intensity variations that can not be corrected .
	manualset3
177226	6	410985	13	NULL	NULL	0	NULL	RF penetration effects 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method may fail in large imaging objects such as the human trunk at high magnetic field where standing wave and RF penetration effects cause intensity variations that can not be corrected .
	manualset3
177227	7	410985	13	NULL	NULL	0	NULL	intensity variations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method may fail in large imaging objects such as the human trunk at high magnetic field where standing wave and RF penetration effects cause intensity variations that can not be corrected .
	manualset3
177228	1	410986	13	NULL	NULL	0	NULL	method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method of immunofluorescence was used to study location of the basal cell cross-reacting antigen shared by group A streptococcus , and multilayer epithelium of the mucous membrane of the oral cavity , oesophagus , vagina , cervix , urinary bladder , eye conjunctiva , epithelial cells of the mammary and salivary gland ducts of man .
	manualset3
177229	2	410986	13	NULL	NULL	0	NULL	immunofluorescence 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method of immunofluorescence was used to study location of the basal cell cross-reacting antigen shared by group A streptococcus , and multilayer epithelium of the mucous membrane of the oral cavity , oesophagus , vagina , cervix , urinary bladder , eye conjunctiva , epithelial cells of the mammary and salivary gland ducts of man .
	manualset3
177230	3	410986	13	NULL	NULL	0	NULL	location	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method of immunofluorescence was used to study location of the basal cell cross-reacting antigen shared by group A streptococcus , and multilayer epithelium of the mucous membrane of the oral cavity , oesophagus , vagina , cervix , urinary bladder , eye conjunctiva , epithelial cells of the mammary and salivary gland ducts of man .
	manualset3
177231	4	410986	13	NULL	NULL	0	NULL	antigen	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The method of immunofluorescence was used to study location of the basal cell cross-reacting antigen shared by group A streptococcus , and multilayer epithelium of the mucous membrane of the oral cavity , oesophagus , vagina , cervix , urinary bladder , eye conjunctiva , epithelial cells of the mammary and salivary gland ducts of man .
	manualset3
177232	5	410986	13	NULL	NULL	0	NULL	group A streptococcus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The method of immunofluorescence was used to study location of the basal cell cross-reacting antigen shared by group A streptococcus , and multilayer epithelium of the mucous membrane of the oral cavity , oesophagus , vagina , cervix , urinary bladder , eye conjunctiva , epithelial cells of the mammary and salivary gland ducts of man .
	manualset3
177233	6	410986	13	NULL	NULL	0	NULL	multilayer epithelium	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The method of immunofluorescence was used to study location of the basal cell cross-reacting antigen shared by group A streptococcus , and multilayer epithelium of the mucous membrane of the oral cavity , oesophagus , vagina , cervix , urinary bladder , eye conjunctiva , epithelial cells of the mammary and salivary gland ducts of man .
	manualset3
177234	7	410986	13	NULL	NULL	0	NULL	mucous membrane	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The method of immunofluorescence was used to study location of the basal cell cross-reacting antigen shared by group A streptococcus , and multilayer epithelium of the mucous membrane of the oral cavity , oesophagus , vagina , cervix , urinary bladder , eye conjunctiva , epithelial cells of the mammary and salivary gland ducts of man .
	manualset3
177235	8	410986	13	NULL	NULL	0	NULL	oral cavity	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The method of immunofluorescence was used to study location of the basal cell cross-reacting antigen shared by group A streptococcus , and multilayer epithelium of the mucous membrane of the oral cavity , oesophagus , vagina , cervix , urinary bladder , eye conjunctiva , epithelial cells of the mammary and salivary gland ducts of man .
	manualset3
177236	9	410986	13	NULL	NULL	0	NULL	oesophagus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The method of immunofluorescence was used to study location of the basal cell cross-reacting antigen shared by group A streptococcus , and multilayer epithelium of the mucous membrane of the oral cavity , oesophagus , vagina , cervix , urinary bladder , eye conjunctiva , epithelial cells of the mammary and salivary gland ducts of man .
	manualset3
177237	10	410986	13	NULL	NULL	0	NULL	vagina 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The method of immunofluorescence was used to study location of the basal cell cross-reacting antigen shared by group A streptococcus , and multilayer epithelium of the mucous membrane of the oral cavity , oesophagus , vagina , cervix , urinary bladder , eye conjunctiva , epithelial cells of the mammary and salivary gland ducts of man .
	manualset3
177238	11	410986	13	NULL	NULL	0	NULL	cervix	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The method of immunofluorescence was used to study location of the basal cell cross-reacting antigen shared by group A streptococcus , and multilayer epithelium of the mucous membrane of the oral cavity , oesophagus , vagina , cervix , urinary bladder , eye conjunctiva , epithelial cells of the mammary and salivary gland ducts of man .
	manualset3
177239	12	410986	13	NULL	NULL	0	NULL	urinary bladder 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The method of immunofluorescence was used to study location of the basal cell cross-reacting antigen shared by group A streptococcus , and multilayer epithelium of the mucous membrane of the oral cavity , oesophagus , vagina , cervix , urinary bladder , eye conjunctiva , epithelial cells of the mammary and salivary gland ducts of man .
	manualset3
177240	13	410986	13	NULL	NULL	0	NULL	eye conjunctiva	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The method of immunofluorescence was used to study location of the basal cell cross-reacting antigen shared by group A streptococcus , and multilayer epithelium of the mucous membrane of the oral cavity , oesophagus , vagina , cervix , urinary bladder , eye conjunctiva , epithelial cells of the mammary and salivary gland ducts of man .
	manualset3
177241	14	410986	13	NULL	NULL	0	NULL	epithelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The method of immunofluorescence was used to study location of the basal cell cross-reacting antigen shared by group A streptococcus , and multilayer epithelium of the mucous membrane of the oral cavity , oesophagus , vagina , cervix , urinary bladder , eye conjunctiva , epithelial cells of the mammary and salivary gland ducts of man .
	manualset3
177242	15	410986	13	NULL	NULL	0	NULL	mammary gland ducts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The method of immunofluorescence was used to study location of the basal cell cross-reacting antigen shared by group A streptococcus , and multilayer epithelium of the mucous membrane of the oral cavity , oesophagus , vagina , cervix , urinary bladder , eye conjunctiva , epithelial cells of the mammary and salivary gland ducts of man .
	manualset3
177243	16	410986	13	NULL	NULL	0	NULL	salivary gland ducts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The method of immunofluorescence was used to study location of the basal cell cross-reacting antigen shared by group A streptococcus , and multilayer epithelium of the mucous membrane of the oral cavity , oesophagus , vagina , cervix , urinary bladder , eye conjunctiva , epithelial cells of the mammary and salivary gland ducts of man .
	manualset3
177244	17	410986	13	NULL	NULL	0	NULL	man	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The method of immunofluorescence was used to study location of the basal cell cross-reacting antigen shared by group A streptococcus , and multilayer epithelium of the mucous membrane of the oral cavity , oesophagus , vagina , cervix , urinary bladder , eye conjunctiva , epithelial cells of the mammary and salivary gland ducts of man .
	manualset3
177256	1	410987	13	NULL	NULL	0	NULL	method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method uses a novel off-line precalibration procedure for spectral bleed-through correction based on the acquisition of reference reflection images , which simplifies the method and reduces variability .
	manualset3
177257	2	410987	13	NULL	NULL	0	NULL	novel off-line precalibration procedure	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The method uses a novel off-line precalibration procedure for spectral bleed-through correction based on the acquisition of reference reflection images , which simplifies the method and reduces variability .
	manualset3
177258	3	410987	13	NULL	NULL	0	NULL	pectral bleed-through correction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method uses a novel off-line precalibration procedure for spectral bleed-through correction based on the acquisition of reference reflection images , which simplifies the method and reduces variability .
	manualset3
177259	4	410987	13	NULL	NULL	0	NULL	 acquisition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method uses a novel off-line precalibration procedure for spectral bleed-through correction based on the acquisition of reference reflection images , which simplifies the method and reduces variability .
	manualset3
177260	5	410987	13	NULL	NULL	0	NULL	reference reflection images	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The method uses a novel off-line precalibration procedure for spectral bleed-through correction based on the acquisition of reference reflection images , which simplifies the method and reduces variability .
	manualset3
177261	6	410987	13	NULL	NULL	0	NULL	 method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method uses a novel off-line precalibration procedure for spectral bleed-through correction based on the acquisition of reference reflection images , which simplifies the method and reduces variability .
	manualset3
177262	7	410987	13	NULL	NULL	0	NULL	variability 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method uses a novel off-line precalibration procedure for spectral bleed-through correction based on the acquisition of reference reflection images , which simplifies the method and reduces variability .
	manualset3
177263	1	410988	13	NULL	NULL	0	NULL	method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was based on the determination of chemiluminescence formed by the reaction of a luminol-ferricyanide mixture in alkaline medium with hydrogen peroxide which is one of the metabolic products of histamine and N tau-methylhistamine formed by diamine oxidase .
	manualset3
177264	2	410988	13	NULL	NULL	0	NULL	determination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was based on the determination of chemiluminescence formed by the reaction of a luminol-ferricyanide mixture in alkaline medium with hydrogen peroxide which is one of the metabolic products of histamine and N tau-methylhistamine formed by diamine oxidase .
	manualset3
177265	3	410988	13	NULL	NULL	0	NULL	chemiluminescence 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was based on the determination of chemiluminescence formed by the reaction of a luminol-ferricyanide mixture in alkaline medium with hydrogen peroxide which is one of the metabolic products of histamine and N tau-methylhistamine formed by diamine oxidase .
	manualset3
177266	4	410988	13	NULL	NULL	0	NULL	reaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was based on the determination of chemiluminescence formed by the reaction of a luminol-ferricyanide mixture in alkaline medium with hydrogen peroxide which is one of the metabolic products of histamine and N tau-methylhistamine formed by diamine oxidase .
	manualset3
177267	5	410988	13	NULL	NULL	0	NULL	 luminol-ferricyanide mixture 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was based on the determination of chemiluminescence formed by the reaction of a luminol-ferricyanide mixture in alkaline medium with hydrogen peroxide which is one of the metabolic products of histamine and N tau-methylhistamine formed by diamine oxidase .
	manualset3
177268	6	410988	13	NULL	NULL	0	NULL	alkaline medium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was based on the determination of chemiluminescence formed by the reaction of a luminol-ferricyanide mixture in alkaline medium with hydrogen peroxide which is one of the metabolic products of histamine and N tau-methylhistamine formed by diamine oxidase .
	manualset3
177269	7	410988	13	NULL	NULL	0	NULL	hydrogen peroxide 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was based on the determination of chemiluminescence formed by the reaction of a luminol-ferricyanide mixture in alkaline medium with hydrogen peroxide which is one of the metabolic products of histamine and N tau-methylhistamine formed by diamine oxidase .
	manualset3
177270	8	410988	13	NULL	NULL	0	NULL	metabolic products	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was based on the determination of chemiluminescence formed by the reaction of a luminol-ferricyanide mixture in alkaline medium with hydrogen peroxide which is one of the metabolic products of histamine and N tau-methylhistamine formed by diamine oxidase .
	manualset3
177271	9	410988	13	NULL	NULL	0	NULL	 histamine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was based on the determination of chemiluminescence formed by the reaction of a luminol-ferricyanide mixture in alkaline medium with hydrogen peroxide which is one of the metabolic products of histamine and N tau-methylhistamine formed by diamine oxidase .
	manualset3
177272	10	410988	13	NULL	NULL	0	NULL	N tau-methylhistamine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was based on the determination of chemiluminescence formed by the reaction of a luminol-ferricyanide mixture in alkaline medium with hydrogen peroxide which is one of the metabolic products of histamine and N tau-methylhistamine formed by diamine oxidase .
	manualset3
177273	11	410988	13	NULL	NULL	0	NULL	diamine oxidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was based on the determination of chemiluminescence formed by the reaction of a luminol-ferricyanide mixture in alkaline medium with hydrogen peroxide which is one of the metabolic products of histamine and N tau-methylhistamine formed by diamine oxidase .
	manualset3
177274	1	410989	13	NULL	NULL	0	NULL	type III collagen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A type III collagen Gly559 to Arg helix mutation in Ehler 's - Danlos syndrome type IV .
	manualset3
177275	2	410989	13	NULL	NULL	0	NULL	Gly559 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A type III collagen Gly559 to Arg helix mutation in Ehler 's - Danlos syndrome type IV .
	manualset3
177276	3	410989	13	NULL	NULL	0	NULL	Arg helix mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A type III collagen Gly559 to Arg helix mutation in Ehler 's - Danlos syndrome type IV .
	manualset3
177277	4	410989	13	NULL	NULL	0	NULL	Ehler 's - Danlos syndrome type IV	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A type III collagen Gly559 to Arg helix mutation in Ehler 's - Danlos syndrome type IV .
	manualset3
177278	1	410990	13	NULL	NULL	0	NULL	 method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was evaluated statistically and under optimized conditions , the detection limits for the analytes were 0.074 and 0.061 ng/mL for B1 and B2 respectively .
	manualset3
177279	2	410990	13	NULL	NULL	0	NULL	conditions	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was evaluated statistically and under optimized conditions , the detection limits for the analytes were 0.074 and 0.061 ng/mL for B1 and B2 respectively .
	manualset3
177280	3	410990	13	NULL	NULL	0	NULL	detection limits	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was evaluated statistically and under optimized conditions , the detection limits for the analytes were 0.074 and 0.061 ng/mL for B1 and B2 respectively .
	manualset3
177281	4	410990	13	NULL	NULL	0	NULL	analytes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was evaluated statistically and under optimized conditions , the detection limits for the analytes were 0.074 and 0.061 ng/mL for B1 and B2 respectively .
	manualset3
177282	5	410990	13	NULL	NULL	0	NULL	0.074 ng/mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was evaluated statistically and under optimized conditions , the detection limits for the analytes were 0.074 and 0.061 ng/mL for B1 and B2 respectively .
	manualset3
177283	6	410990	13	NULL	NULL	0	NULL	 0.061 ng/mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was evaluated statistically and under optimized conditions , the detection limits for the analytes were 0.074 and 0.061 ng/mL for B1 and B2 respectively .
	manualset3
177284	7	410990	13	NULL	NULL	0	NULL	B1	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was evaluated statistically and under optimized conditions , the detection limits for the analytes were 0.074 and 0.061 ng/mL for B1 and B2 respectively .
	manualset3
177285	8	410990	13	NULL	NULL	0	NULL	B2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was evaluated statistically and under optimized conditions , the detection limits for the analytes were 0.074 and 0.061 ng/mL for B1 and B2 respectively .
	manualset3
177286	1	410991	13	NULL	NULL	0	NULL	 method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was used to quantitate the amount of SP produced upon irradiation of B. subtilis spores and to monitor repair of SP in vivo by the enzyme SP lyase during spore germination .
	manualset3
177287	2	410991	13	NULL	NULL	0	NULL	amount	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was used to quantitate the amount of SP produced upon irradiation of B. subtilis spores and to monitor repair of SP in vivo by the enzyme SP lyase during spore germination .
	manualset3
177288	3	410991	13	NULL	NULL	0	NULL	SP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was used to quantitate the amount of SP produced upon irradiation of B. subtilis spores and to monitor repair of SP in vivo by the enzyme SP lyase during spore germination .
	manualset3
177289	4	410991	13	NULL	NULL	0	NULL	irradiation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was used to quantitate the amount of SP produced upon irradiation of B. subtilis spores and to monitor repair of SP in vivo by the enzyme SP lyase during spore germination .
	manualset3
177290	5	410991	13	NULL	NULL	0	NULL	B. subtilis spores	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was used to quantitate the amount of SP produced upon irradiation of B. subtilis spores and to monitor repair of SP in vivo by the enzyme SP lyase during spore germination .
	manualset3
177291	6	410991	13	NULL	NULL	0	NULL	SP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was used to quantitate the amount of SP produced upon irradiation of B. subtilis spores and to monitor repair of SP in vivo by the enzyme SP lyase during spore germination .
	manualset3
177292	7	410991	13	NULL	NULL	0	NULL	enzyme SP lyase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was used to quantitate the amount of SP produced upon irradiation of B. subtilis spores and to monitor repair of SP in vivo by the enzyme SP lyase during spore germination .
	manualset3
177293	8	410991	13	NULL	NULL	0	NULL	spore germination 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was used to quantitate the amount of SP produced upon irradiation of B. subtilis spores and to monitor repair of SP in vivo by the enzyme SP lyase during spore germination .
	manualset3
200342	9	410991	13	NULL	NULL	0	NULL	repair 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was used to quantitate the amount of SP produced upon irradiation of B. subtilis spores and to monitor repair of SP in vivo by the enzyme SP lyase during spore germination .
	manualset3
177294	1	410992	13	NULL	NULL	0	NULL	method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was validated in terms of selectivity , recoveries , calibration , precision and accuracy as well as matrix effects .
	manualset3
177295	2	410992	13	NULL	NULL	0	NULL	selectivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was validated in terms of selectivity , recoveries , calibration , precision and accuracy as well as matrix effects .
	manualset3
177296	3	410992	13	NULL	NULL	0	NULL	recoveries	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was validated in terms of selectivity , recoveries , calibration , precision and accuracy as well as matrix effects .
	manualset3
177297	4	410992	13	NULL	NULL	0	NULL	calibration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was validated in terms of selectivity , recoveries , calibration , precision and accuracy as well as matrix effects .
	manualset3
177298	5	410992	13	NULL	NULL	0	NULL	precision	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was validated in terms of selectivity , recoveries , calibration , precision and accuracy as well as matrix effects .
	manualset3
177299	6	410992	13	NULL	NULL	0	NULL	accuracy	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was validated in terms of selectivity , recoveries , calibration , precision and accuracy as well as matrix effects .
	manualset3
177300	7	410992	13	NULL	NULL	0	NULL	matrix effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was validated in terms of selectivity , recoveries , calibration , precision and accuracy as well as matrix effects .
	manualset3
177301	8	410992	13	NULL	NULL	0	NULL	terms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was validated in terms of selectivity , recoveries , calibration , precision and accuracy as well as matrix effects .
	manualset3
177302	1	410993	13	NULL	NULL	0	NULL	method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was validated with respect to linearity , precision , accuracy , selectivity , specificity and ruggedness .
	manualset3
177303	2	410993	13	NULL	NULL	0	NULL	respect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was validated with respect to linearity , precision , accuracy , selectivity , specificity and ruggedness .
	manualset3
177304	3	410993	13	NULL	NULL	0	NULL	linearity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was validated with respect to linearity , precision , accuracy , selectivity , specificity and ruggedness .
	manualset3
177305	4	410993	13	NULL	NULL	0	NULL	precision	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was validated with respect to linearity , precision , accuracy , selectivity , specificity and ruggedness .
	manualset3
177306	5	410993	13	NULL	NULL	0	NULL	accuracy	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was validated with respect to linearity , precision , accuracy , selectivity , specificity and ruggedness .
	manualset3
177307	6	410993	13	NULL	NULL	0	NULL	selectivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was validated with respect to linearity , precision , accuracy , selectivity , specificity and ruggedness .
	manualset3
177308	7	410993	13	NULL	NULL	0	NULL	specificity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was validated with respect to linearity , precision , accuracy , selectivity , specificity and ruggedness .
	manualset3
177309	8	410993	13	NULL	NULL	0	NULL	ruggedness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method was validated with respect to linearity , precision , accuracy , selectivity , specificity and ruggedness .
	manualset3
177310	1	410994	13	NULL	NULL	0	NULL	methodology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The methodology developed here constitutes a sensitive analytical tool to study enzymes requiring long equilibration times .
	manualset3
177311	2	410994	13	NULL	NULL	0	NULL	sensitive analytical tool 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The methodology developed here constitutes a sensitive analytical tool to study enzymes requiring long equilibration times .
	manualset3
177312	3	410994	13	NULL	NULL	0	NULL	enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The methodology developed here constitutes a sensitive analytical tool to study enzymes requiring long equilibration times .
	manualset3
177313	4	410994	13	NULL	NULL	0	NULL	equilibration times	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The methodology developed here constitutes a sensitive analytical tool to study enzymes requiring long equilibration times .
	manualset3
177324	1	410995	13	NULL	NULL	0	NULL	methodology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The methodology includes focus-group discussions , an in-depth study of 25 families , and ethnographic observation .
	manualset3
177330	2	410995	13	NULL	NULL	0	NULL	focus-group discussions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The methodology includes focus-group discussions , an in-depth study of 25 families , and ethnographic observation .
	manualset3
177331	3	410995	13	NULL	NULL	0	NULL	25 families 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The methodology includes focus-group discussions , an in-depth study of 25 families , and ethnographic observation .
	manualset3
177332	4	410995	13	NULL	NULL	0	NULL	 ethnographic observation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The methodology includes focus-group discussions , an in-depth study of 25 families , and ethnographic observation .
	manualset3
177346	5	410995	13	NULL	NULL	0	NULL	in-depth study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The methodology includes focus-group discussions , an in-depth study of 25 families , and ethnographic observation .
	manualset3
177355	1	410996	13	NULL	NULL	0	NULL	 methods	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The methods of implementation will be described as well as the attitudes of the effectiveness of the strategy based upon participant satisfaction .
	manualset3
177356	2	410996	13	NULL	NULL	0	NULL	implementation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The methods of implementation will be described as well as the attitudes of the effectiveness of the strategy based upon participant satisfaction .
	manualset3
177357	3	410996	13	NULL	NULL	0	NULL	attitudes 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The methods of implementation will be described as well as the attitudes of the effectiveness of the strategy based upon participant satisfaction .
	manualset3
177358	4	410996	13	NULL	NULL	0	NULL	 effectiveness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The methods of implementation will be described as well as the attitudes of the effectiveness of the strategy based upon participant satisfaction .
	manualset3
177359	5	410996	13	NULL	NULL	0	NULL	strategy	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The methods of implementation will be described as well as the attitudes of the effectiveness of the strategy based upon participant satisfaction .
	manualset3
177360	6	410996	13	NULL	NULL	0	NULL	participant	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The methods of implementation will be described as well as the attitudes of the effectiveness of the strategy based upon participant satisfaction .
	manualset3
177361	7	410996	13	NULL	NULL	0	NULL	satisfaction 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The methods of implementation will be described as well as the attitudes of the effectiveness of the strategy based upon participant satisfaction .
	manualset3
177363	1	410997	13	NULL	NULL	0	NULL	methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The methods showed excellent linearity ( r2 ) 0.99 ) over the concentration ranges tested ( 0.25-5 .0 nmoles of TESG ; 0.125-18 .75 nmoles of 8HOQG and 0.125-12 .5 nmoles of 4MUG ) , good precision and accuracy ( RSD & lt ; 2.5 % ) .
	manualset3
177366	2	410997	13	NULL	NULL	0	NULL	linearity 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The methods showed excellent linearity ( r2 ) 0.99 ) over the concentration ranges tested ( 0.25-5 .0 nmoles of TESG ; 0.125-18 .75 nmoles of 8HOQG and 0.125-12 .5 nmoles of 4MUG ) , good precision and accuracy ( RSD & lt ; 2.5 % ) .
	manualset3
177368	3	410997	13	NULL	NULL	0	NULL	( r2 ) 0.99 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The methods showed excellent linearity ( r2 ) 0.99 ) over the concentration ranges tested ( 0.25-5 .0 nmoles of TESG ; 0.125-18 .75 nmoles of 8HOQG and 0.125-12 .5 nmoles of 4MUG ) , good precision and accuracy ( RSD & lt ; 2.5 % ) .
	manualset3
177369	4	410997	13	NULL	NULL	0	NULL	concentration ranges	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The methods showed excellent linearity ( r2 ) 0.99 ) over the concentration ranges tested ( 0.25-5 .0 nmoles of TESG ; 0.125-18 .75 nmoles of 8HOQG and 0.125-12 .5 nmoles of 4MUG ) , good precision and accuracy ( RSD & lt ; 2.5 % ) .
	manualset3
177370	5	410997	13	NULL	NULL	0	NULL	0.25-5 .0 nmoles	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The methods showed excellent linearity ( r2 ) 0.99 ) over the concentration ranges tested ( 0.25-5 .0 nmoles of TESG ; 0.125-18 .75 nmoles of 8HOQG and 0.125-12 .5 nmoles of 4MUG ) , good precision and accuracy ( RSD & lt ; 2.5 % ) .
	manualset3
177371	6	410997	13	NULL	NULL	0	NULL	TESG	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The methods showed excellent linearity ( r2 ) 0.99 ) over the concentration ranges tested ( 0.25-5 .0 nmoles of TESG ; 0.125-18 .75 nmoles of 8HOQG and 0.125-12 .5 nmoles of 4MUG ) , good precision and accuracy ( RSD & lt ; 2.5 % ) .
	manualset3
177372	7	410997	13	NULL	NULL	0	NULL	0.125-18 .75 nmoles	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The methods showed excellent linearity ( r2 ) 0.99 ) over the concentration ranges tested ( 0.25-5 .0 nmoles of TESG ; 0.125-18 .75 nmoles of 8HOQG and 0.125-12 .5 nmoles of 4MUG ) , good precision and accuracy ( RSD & lt ; 2.5 % ) .
	manualset3
177373	8	410997	13	NULL	NULL	0	NULL	8HOQG 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The methods showed excellent linearity ( r2 ) 0.99 ) over the concentration ranges tested ( 0.25-5 .0 nmoles of TESG ; 0.125-18 .75 nmoles of 8HOQG and 0.125-12 .5 nmoles of 4MUG ) , good precision and accuracy ( RSD & lt ; 2.5 % ) .
	manualset3
177374	9	410997	13	NULL	NULL	0	NULL	0.125-12 .5 nmoles	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The methods showed excellent linearity ( r2 ) 0.99 ) over the concentration ranges tested ( 0.25-5 .0 nmoles of TESG ; 0.125-18 .75 nmoles of 8HOQG and 0.125-12 .5 nmoles of 4MUG ) , good precision and accuracy ( RSD & lt ; 2.5 % ) .
	manualset3
177375	10	410997	13	NULL	NULL	0	NULL	4MUG	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The methods showed excellent linearity ( r2 ) 0.99 ) over the concentration ranges tested ( 0.25-5 .0 nmoles of TESG ; 0.125-18 .75 nmoles of 8HOQG and 0.125-12 .5 nmoles of 4MUG ) , good precision and accuracy ( RSD & lt ; 2.5 % ) .
	manualset3
177376	11	410997	13	NULL	NULL	0	NULL	precision 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The methods showed excellent linearity ( r2 ) 0.99 ) over the concentration ranges tested ( 0.25-5 .0 nmoles of TESG ; 0.125-18 .75 nmoles of 8HOQG and 0.125-12 .5 nmoles of 4MUG ) , good precision and accuracy ( RSD & lt ; 2.5 % ) .
	manualset3
177377	12	410997	13	NULL	NULL	0	NULL	accuracy 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The methods showed excellent linearity ( r2 ) 0.99 ) over the concentration ranges tested ( 0.25-5 .0 nmoles of TESG ; 0.125-18 .75 nmoles of 8HOQG and 0.125-12 .5 nmoles of 4MUG ) , good precision and accuracy ( RSD & lt ; 2.5 % ) .
	manualset3
177378	13	410997	13	NULL	NULL	0	NULL	RSD & lt ; 2.5 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The methods showed excellent linearity ( r2 ) 0.99 ) over the concentration ranges tested ( 0.25-5 .0 nmoles of TESG ; 0.125-18 .75 nmoles of 8HOQG and 0.125-12 .5 nmoles of 4MUG ) , good precision and accuracy ( RSD & lt ; 2.5 % ) .
	manualset3
177379	1	410998	13	NULL	NULL	0	NULL	methoxy methyl group	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The methoxy methyl group of MTBE was oxidized to formaldehyde and ultimately to CO2 .
	manualset3
177380	2	410998	13	NULL	NULL	0	NULL	MTBE	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The methoxy methyl group of MTBE was oxidized to formaldehyde and ultimately to CO2 .
	manualset3
177381	3	410998	13	NULL	NULL	0	NULL	formaldehyde 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The methoxy methyl group of MTBE was oxidized to formaldehyde and ultimately to CO2 .
	manualset3
177382	4	410998	13	NULL	NULL	0	NULL	CO2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The methoxy methyl group of MTBE was oxidized to formaldehyde and ultimately to CO2 .
	manualset3
177383	1	410999	13	NULL	NULL	0	NULL	methyl substitution 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The methyl substitution at positions C9 or C10 increased the T antigen expression of adenovirus infected cells .
	manualset3
177384	2	410999	13	NULL	NULL	0	NULL	positions C9	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The methyl substitution at positions C9 or C10 increased the T antigen expression of adenovirus infected cells .
	manualset3
177385	3	410999	13	NULL	NULL	0	NULL	positions C10	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The methyl substitution at positions C9 or C10 increased the T antigen expression of adenovirus infected cells .
	manualset3
177386	4	410999	13	NULL	NULL	0	NULL	T antigen expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The methyl substitution at positions C9 or C10 increased the T antigen expression of adenovirus infected cells .
	manualset3
177387	5	410999	13	NULL	NULL	0	NULL	 adenovirus infected cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The methyl substitution at positions C9 or C10 increased the T antigen expression of adenovirus infected cells .
	manualset3
177395	1	411000	13	NULL	NULL	0	NULL	microbiology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The microbiology and clinical features of empyema were studied retrospectively in 197 patients whose specimens yielded bacterial growth after inoculation for aerobic and anaerobic bacteria .
	manualset3
177396	2	411000	13	NULL	NULL	0	NULL	clinical features	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The microbiology and clinical features of empyema were studied retrospectively in 197 patients whose specimens yielded bacterial growth after inoculation for aerobic and anaerobic bacteria .
	manualset3
177397	3	411000	13	NULL	NULL	0	NULL	empyema 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The microbiology and clinical features of empyema were studied retrospectively in 197 patients whose specimens yielded bacterial growth after inoculation for aerobic and anaerobic bacteria .
	manualset3
177398	4	411000	13	NULL	NULL	0	NULL	197 patients	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The microbiology and clinical features of empyema were studied retrospectively in 197 patients whose specimens yielded bacterial growth after inoculation for aerobic and anaerobic bacteria .
	manualset3
177401	5	411000	13	NULL	NULL	0	NULL	specimens	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The microbiology and clinical features of empyema were studied retrospectively in 197 patients whose specimens yielded bacterial growth after inoculation for aerobic and anaerobic bacteria .
	manualset3
177404	6	411000	13	NULL	NULL	0	NULL	bacterial growth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The microbiology and clinical features of empyema were studied retrospectively in 197 patients whose specimens yielded bacterial growth after inoculation for aerobic and anaerobic bacteria .
	manualset3
177406	7	411000	13	NULL	NULL	0	NULL	inoculation	MedicalProcedureOrDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The microbiology and clinical features of empyema were studied retrospectively in 197 patients whose specimens yielded bacterial growth after inoculation for aerobic and anaerobic bacteria .
	manualset3
177407	8	411000	13	NULL	NULL	0	NULL	aerobic bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The microbiology and clinical features of empyema were studied retrospectively in 197 patients whose specimens yielded bacterial growth after inoculation for aerobic and anaerobic bacteria .
	manualset3
177408	9	411000	13	NULL	NULL	0	NULL	anaerobic bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The microbiology and clinical features of empyema were studied retrospectively in 197 patients whose specimens yielded bacterial growth after inoculation for aerobic and anaerobic bacteria .
	manualset3
177420	1	411001	13	NULL	NULL	NULL	NULL	microdialysate samples 	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The microdialysate samples , obtained from the probe outlet , can be analyzed using high-performance liquid chromatography with electrochemical detection for the quantification of oxidizable molecules recovered from the extracellular space .
	manualset3
177421	2	411001	13	NULL	NULL	0	NULL	 probe outlet	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The microdialysate samples , obtained from the probe outlet , can be analyzed using high-performance liquid chromatography with electrochemical detection for the quantification of oxidizable molecules recovered from the extracellular space .
	manualset3
177422	3	411001	13	NULL	NULL	0	NULL	high-performance liquid chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The microdialysate samples , obtained from the probe outlet , can be analyzed using high-performance liquid chromatography with electrochemical detection for the quantification of oxidizable molecules recovered from the extracellular space .
	manualset3
177423	4	411001	13	NULL	NULL	0	NULL	electrochemical detection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The microdialysate samples , obtained from the probe outlet , can be analyzed using high-performance liquid chromatography with electrochemical detection for the quantification of oxidizable molecules recovered from the extracellular space .
	manualset3
177424	5	411001	13	NULL	NULL	0	NULL	quantification 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The microdialysate samples , obtained from the probe outlet , can be analyzed using high-performance liquid chromatography with electrochemical detection for the quantification of oxidizable molecules recovered from the extracellular space .
	manualset3
177425	6	411001	13	NULL	NULL	0	NULL	oxidizable molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The microdialysate samples , obtained from the probe outlet , can be analyzed using high-performance liquid chromatography with electrochemical detection for the quantification of oxidizable molecules recovered from the extracellular space .
	manualset3
177426	7	411001	13	NULL	NULL	0	NULL	extracellular space	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The microdialysate samples , obtained from the probe outlet , can be analyzed using high-performance liquid chromatography with electrochemical detection for the quantification of oxidizable molecules recovered from the extracellular space .
	manualset3
177430	1	411002	13	NULL	NULL	0	NULL	microphonics	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The microphonics of lateral line hair cells of orbiter , mercury , and gemini larvae are absent or strongly reduced .
	manualset3
177431	2	411002	13	NULL	NULL	0	NULL	lateral line hair cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The microphonics of lateral line hair cells of orbiter , mercury , and gemini larvae are absent or strongly reduced .
	manualset3
177433	3	411002	13	NULL	NULL	0	NULL	orbiter larvae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The microphonics of lateral line hair cells of orbiter , mercury , and gemini larvae are absent or strongly reduced .
	manualset3
177435	4	411002	13	NULL	NULL	0	NULL	mercury larvae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The microphonics of lateral line hair cells of orbiter , mercury , and gemini larvae are absent or strongly reduced .
	manualset3
177437	5	411002	13	NULL	NULL	0	NULL	gemini larvae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The microphonics of lateral line hair cells of orbiter , mercury , and gemini larvae are absent or strongly reduced .
	manualset3
177439	1	411003	13	NULL	NULL	0	NULL	microscopic morphology	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The microscopic morphology and size of the flocculates was dependent on the molecular structure of the polymer , especially ether groups on the polymer side chain .
	manualset3
177441	2	411003	13	NULL	NULL	0	NULL	size 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The microscopic morphology and size of the flocculates was dependent on the molecular structure of the polymer , especially ether groups on the polymer side chain .
	manualset3
177442	3	411003	13	NULL	NULL	0	NULL	flocculates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The microscopic morphology and size of the flocculates was dependent on the molecular structure of the polymer , especially ether groups on the polymer side chain .
	manualset3
177443	4	411003	13	NULL	NULL	NULL	NULL	molecular structure	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The microscopic morphology and size of the flocculates was dependent on the molecular structure of the polymer , especially ether groups on the polymer side chain .
	manualset3
177444	5	411003	13	NULL	NULL	0	NULL	polymer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The microscopic morphology and size of the flocculates was dependent on the molecular structure of the polymer , especially ether groups on the polymer side chain .
	manualset3
177445	6	411003	13	NULL	NULL	0	NULL	ether groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The microscopic morphology and size of the flocculates was dependent on the molecular structure of the polymer , especially ether groups on the polymer side chain .
	manualset3
177446	7	411003	13	NULL	NULL	0	NULL	 polymer side chain 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The microscopic morphology and size of the flocculates was dependent on the molecular structure of the polymer , especially ether groups on the polymer side chain .
	manualset3
177484	1	411004	13	NULL	NULL	0	NULL	microsphere-captured probe	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The microsphere-captured probe was then released by heat denaturation and added into unmodified gold nanoparticle ( AuNP ) solution .
	manualset3
177485	2	411004	13	NULL	NULL	0	NULL	heat denaturation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The microsphere-captured probe was then released by heat denaturation and added into unmodified gold nanoparticle ( AuNP ) solution .
	manualset3
177486	3	411004	13	NULL	NULL	0	NULL	gold nanoparticle ( AuNP ) solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The microsphere-captured probe was then released by heat denaturation and added into unmodified gold nanoparticle ( AuNP ) solution .
	manualset3
177487	1	411005	13	NULL	NULL	0	NULL	microwave drill	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The microwave drill uses a near-field focused energy ( typically , power under approximately 200 W at 2.45-GHz frequency ) in order to penetrate bone in a drilling speed of approximately 1 mm/s .
	manualset3
177488	2	411005	13	NULL	NULL	0	NULL	energy	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The microwave drill uses a near-field focused energy ( typically , power under approximately 200 W at 2.45-GHz frequency ) in order to penetrate bone in a drilling speed of approximately 1 mm/s .
	manualset3
177489	3	411005	13	NULL	NULL	0	NULL	power	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The microwave drill uses a near-field focused energy ( typically , power under approximately 200 W at 2.45-GHz frequency ) in order to penetrate bone in a drilling speed of approximately 1 mm/s .
	manualset3
177490	4	411005	13	NULL	NULL	0	NULL	200 W	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The microwave drill uses a near-field focused energy ( typically , power under approximately 200 W at 2.45-GHz frequency ) in order to penetrate bone in a drilling speed of approximately 1 mm/s .
	manualset3
177491	5	411005	13	NULL	NULL	0	NULL	2.45-GHz frequency	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The microwave drill uses a near-field focused energy ( typically , power under approximately 200 W at 2.45-GHz frequency ) in order to penetrate bone in a drilling speed of approximately 1 mm/s .
	manualset3
177492	6	411005	13	NULL	NULL	0	NULL	bone	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The microwave drill uses a near-field focused energy ( typically , power under approximately 200 W at 2.45-GHz frequency ) in order to penetrate bone in a drilling speed of approximately 1 mm/s .
	manualset3
177493	7	411005	13	NULL	NULL	0	NULL	speed 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The microwave drill uses a near-field focused energy ( typically , power under approximately 200 W at 2.45-GHz frequency ) in order to penetrate bone in a drilling speed of approximately 1 mm/s .
	manualset3
177494	8	411005	13	NULL	NULL	0	NULL	1 mm/s	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The microwave drill uses a near-field focused energy ( typically , power under approximately 200 W at 2.45-GHz frequency ) in order to penetrate bone in a drilling speed of approximately 1 mm/s .
	manualset3
177495	1	411006	13	NULL	NULL	0	NULL	midbody	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The midbody is an electron-dense structure that forms between two dividing daughter cells , and a midbody remnant is left after completion of cell separation .
	manualset3
177496	2	411006	13	NULL	NULL	0	NULL	electron-dense structure	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The midbody is an electron-dense structure that forms between two dividing daughter cells , and a midbody remnant is left after completion of cell separation .
	manualset3
177497	3	411006	13	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The midbody is an electron-dense structure that forms between two dividing daughter cells , and a midbody remnant is left after completion of cell separation .
	manualset3
177498	4	411006	13	NULL	NULL	0	NULL	daughter cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The midbody is an electron-dense structure that forms between two dividing daughter cells , and a midbody remnant is left after completion of cell separation .
	manualset3
177499	5	411006	13	NULL	NULL	0	NULL	midbody remnant	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The midbody is an electron-dense structure that forms between two dividing daughter cells , and a midbody remnant is left after completion of cell separation .
	manualset3
177500	6	411006	13	NULL	NULL	0	NULL	 completion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The midbody is an electron-dense structure that forms between two dividing daughter cells , and a midbody remnant is left after completion of cell separation .
	manualset3
177501	7	411006	13	NULL	NULL	0	NULL	cell separation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The midbody is an electron-dense structure that forms between two dividing daughter cells , and a midbody remnant is left after completion of cell separation .
	manualset3
177502	1	411007	13	NULL	NULL	NULL	NULL	middle finger compartment	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The middle finger compartment of extensor digitorum communis was found to be incapable of isolated contractions and is therefore not recommended as a control site for direct myocontrol prostheses .
	manualset3
177505	2	411007	13	NULL	NULL	0	NULL	extensor digitorum communis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The middle finger compartment of extensor digitorum communis was found to be incapable of isolated contractions and is therefore not recommended as a control site for direct myocontrol prostheses .
	manualset3
177506	3	411007	13	NULL	NULL	0	NULL	contractions 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The middle finger compartment of extensor digitorum communis was found to be incapable of isolated contractions and is therefore not recommended as a control site for direct myocontrol prostheses .
	manualset3
177507	4	411007	13	NULL	NULL	0	NULL	control site 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The middle finger compartment of extensor digitorum communis was found to be incapable of isolated contractions and is therefore not recommended as a control site for direct myocontrol prostheses .
	manualset3
177508	5	411007	13	NULL	NULL	0	NULL	myocontrol prostheses	MedicalProcedureOrDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The middle finger compartment of extensor digitorum communis was found to be incapable of isolated contractions and is therefore not recommended as a control site for direct myocontrol prostheses .
	manualset3
177511	1	411008	13	NULL	NULL	0	NULL	milk WT	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The milk WT was calculated by the Time to Safe Concentration method ( Software WTM 1.4 , EMEA ) .
	manualset3
177513	2	411008	13	NULL	NULL	0	NULL	Time to Safe Concentration method 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The milk WT was calculated by the Time to Safe Concentration method ( Software WTM 1.4 , EMEA ) .
	manualset3
177514	3	411008	13	NULL	NULL	0	NULL	Software WTM 1.4 , EMEA 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The milk WT was calculated by the Time to Safe Concentration method ( Software WTM 1.4 , EMEA ) .
	manualset3
177518	1	411009	13	NULL	NULL	0	NULL	mineral density	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mineral density was reduced in all teeth , including molars and incisors , and in the mandible , and the mineralized tooth volume in incisor and molars , and the mineralized cortical and alveolar bone volume in mandibles were decreased in FGF23 transgenic mice compared with their wild-type littermates .
	manualset3
177519	2	411009	13	NULL	NULL	0	NULL	teeth	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The mineral density was reduced in all teeth , including molars and incisors , and in the mandible , and the mineralized tooth volume in incisor and molars , and the mineralized cortical and alveolar bone volume in mandibles were decreased in FGF23 transgenic mice compared with their wild-type littermates .
	manualset3
177521	3	411009	13	NULL	NULL	0	NULL	molars	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The mineral density was reduced in all teeth , including molars and incisors , and in the mandible , and the mineralized tooth volume in incisor and molars , and the mineralized cortical and alveolar bone volume in mandibles were decreased in FGF23 transgenic mice compared with their wild-type littermates .
	manualset3
177522	4	411009	13	NULL	NULL	0	NULL	incisors	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The mineral density was reduced in all teeth , including molars and incisors , and in the mandible , and the mineralized tooth volume in incisor and molars , and the mineralized cortical and alveolar bone volume in mandibles were decreased in FGF23 transgenic mice compared with their wild-type littermates .
	manualset3
177523	5	411009	13	NULL	NULL	0	NULL	mandible	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The mineral density was reduced in all teeth , including molars and incisors , and in the mandible , and the mineralized tooth volume in incisor and molars , and the mineralized cortical and alveolar bone volume in mandibles were decreased in FGF23 transgenic mice compared with their wild-type littermates .
	manualset3
177524	6	411009	13	NULL	NULL	0	NULL	tooth volume	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mineral density was reduced in all teeth , including molars and incisors , and in the mandible , and the mineralized tooth volume in incisor and molars , and the mineralized cortical and alveolar bone volume in mandibles were decreased in FGF23 transgenic mice compared with their wild-type littermates .
	manualset3
177530	7	411009	13	NULL	NULL	0	NULL	incisor 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The mineral density was reduced in all teeth , including molars and incisors , and in the mandible , and the mineralized tooth volume in incisor and molars , and the mineralized cortical and alveolar bone volume in mandibles were decreased in FGF23 transgenic mice compared with their wild-type littermates .
	manualset3
177532	8	411009	13	NULL	NULL	0	NULL	molars	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The mineral density was reduced in all teeth , including molars and incisors , and in the mandible , and the mineralized tooth volume in incisor and molars , and the mineralized cortical and alveolar bone volume in mandibles were decreased in FGF23 transgenic mice compared with their wild-type littermates .
	manualset3
177536	9	411009	13	NULL	NULL	0	NULL	mineralized cortical bone volume	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mineral density was reduced in all teeth , including molars and incisors , and in the mandible , and the mineralized tooth volume in incisor and molars , and the mineralized cortical and alveolar bone volume in mandibles were decreased in FGF23 transgenic mice compared with their wild-type littermates .
	manualset3
177537	10	411009	13	NULL	NULL	0	NULL	alveolar bone volume	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mineral density was reduced in all teeth , including molars and incisors , and in the mandible , and the mineralized tooth volume in incisor and molars , and the mineralized cortical and alveolar bone volume in mandibles were decreased in FGF23 transgenic mice compared with their wild-type littermates .
	manualset3
177538	11	411009	13	NULL	NULL	0	NULL	mandibles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The mineral density was reduced in all teeth , including molars and incisors , and in the mandible , and the mineralized tooth volume in incisor and molars , and the mineralized cortical and alveolar bone volume in mandibles were decreased in FGF23 transgenic mice compared with their wild-type littermates .
	manualset3
177539	12	411009	13	NULL	NULL	0	NULL	FGF23 transgenic mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The mineral density was reduced in all teeth , including molars and incisors , and in the mandible , and the mineralized tooth volume in incisor and molars , and the mineralized cortical and alveolar bone volume in mandibles were decreased in FGF23 transgenic mice compared with their wild-type littermates .
	manualset3
177540	13	411009	13	NULL	NULL	0	NULL	wild-type littermates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The mineral density was reduced in all teeth , including molars and incisors , and in the mandible , and the mineralized tooth volume in incisor and molars , and the mineralized cortical and alveolar bone volume in mandibles were decreased in FGF23 transgenic mice compared with their wild-type littermates .
	manualset3
177541	1	411010	13	NULL	NULL	0	NULL	minimal interactive regions	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimal interactive regions were mapped to the homeodomain of Nkx-2 .5 and the second zinc finger of GATA-4 .
	manualset3
177542	2	411010	13	NULL	NULL	0	NULL	 homeodomain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimal interactive regions were mapped to the homeodomain of Nkx-2 .5 and the second zinc finger of GATA-4 .
	manualset3
177543	3	411010	13	NULL	NULL	0	NULL	Nkx-2 .5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimal interactive regions were mapped to the homeodomain of Nkx-2 .5 and the second zinc finger of GATA-4 .
	manualset3
177544	4	411010	13	NULL	NULL	0	NULL	 second zinc finger	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimal interactive regions were mapped to the homeodomain of Nkx-2 .5 and the second zinc finger of GATA-4 .
	manualset3
177545	5	411010	13	NULL	NULL	0	NULL	GATA-4 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimal interactive regions were mapped to the homeodomain of Nkx-2 .5 and the second zinc finger of GATA-4 .
	manualset3
177597	1	411011	13	NULL	NULL	0	NULL	unique feature 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A unique feature of DACS is that it permits unbiased evaluation of the chromatin state of regulatory sequences from widely separated genomic loci .
	manualset3
177598	2	411011	13	NULL	NULL	0	NULL	DACS	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A unique feature of DACS is that it permits unbiased evaluation of the chromatin state of regulatory sequences from widely separated genomic loci .
	manualset3
177599	3	411011	13	NULL	NULL	0	NULL	evaluation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A unique feature of DACS is that it permits unbiased evaluation of the chromatin state of regulatory sequences from widely separated genomic loci .
	manualset3
177600	4	411011	13	NULL	NULL	0	NULL	chromatin state	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A unique feature of DACS is that it permits unbiased evaluation of the chromatin state of regulatory sequences from widely separated genomic loci .
	manualset3
177601	5	411011	13	NULL	NULL	0	NULL	regulatory sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A unique feature of DACS is that it permits unbiased evaluation of the chromatin state of regulatory sequences from widely separated genomic loci .
	manualset3
177602	6	411011	13	NULL	NULL	0	NULL	 genomic loci 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A unique feature of DACS is that it permits unbiased evaluation of the chromatin state of regulatory sequences from widely separated genomic loci .
	manualset3
177603	1	411012	13	NULL	NULL	0	NULL	minimal resistance-inducing dose	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimal resistance-inducing dose of the wild type SV40 virus strain was 10 times higher than that of ts A-30 mutant of this virus .
	manualset3
177604	2	411012	13	NULL	NULL	0	NULL	 wild type SV40 virus strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimal resistance-inducing dose of the wild type SV40 virus strain was 10 times higher than that of ts A-30 mutant of this virus .
	manualset3
177605	3	411012	13	NULL	NULL	0	NULL	10 times	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimal resistance-inducing dose of the wild type SV40 virus strain was 10 times higher than that of ts A-30 mutant of this virus .
	manualset3
177606	4	411012	13	NULL	NULL	0	NULL	A-30 mutant 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimal resistance-inducing dose of the wild type SV40 virus strain was 10 times higher than that of ts A-30 mutant of this virus .
	manualset3
177607	5	411012	13	NULL	NULL	0	NULL	virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimal resistance-inducing dose of the wild type SV40 virus strain was 10 times higher than that of ts A-30 mutant of this virus .
	manualset3
177608	1	411013	13	NULL	NULL	0	NULL	follow-up	MedicalProcedureOrDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimum follow-up was 4 years .
	manualset3
177609	2	411013	13	NULL	NULL	0	NULL	4 years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimum follow-up was 4 years .
	manualset3
177610	1	411014	13	NULL	NULL	0	NULL	minimum inhibitory concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimum inhibitory concentrations of the following antibiotics were performed by a liquid micro dilution technic : amoxicillin ( AMX ) , amoxicillin + clavulanic acid ( CL ) , 5 mg/l , ticarcillin ( TIC ) , piperacillin ( PIP ) , cefazolin ( CEZ ) , cefamandole ( CFM ) , cefoperazone ( CFP ) , cefotaxime ( CTX ) , cefotaxime + clavulanic acid 5 mg/l , cefotaxime + sulbactam ( SUL ) 5 mg/l , cefpirome ( CPI ) , ceftazidime ( CAZ ) , azthreonam ( AZT ) , latamoxef ( MOX ) , cefoxitin ( FOX ) , cefotetan ( CTT ) , temocillin ( TMO ) , imipenem ( IMI ) .
	manualset3
177611	2	411014	13	NULL	NULL	0	NULL	antibiotics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimum inhibitory concentrations of the following antibiotics were performed by a liquid micro dilution technic : amoxicillin ( AMX ) , amoxicillin + clavulanic acid ( CL ) , 5 mg/l , ticarcillin ( TIC ) , piperacillin ( PIP ) , cefazolin ( CEZ ) , cefamandole ( CFM ) , cefoperazone ( CFP ) , cefotaxime ( CTX ) , cefotaxime + clavulanic acid 5 mg/l , cefotaxime + sulbactam ( SUL ) 5 mg/l , cefpirome ( CPI ) , ceftazidime ( CAZ ) , azthreonam ( AZT ) , latamoxef ( MOX ) , cefoxitin ( FOX ) , cefotetan ( CTT ) , temocillin ( TMO ) , imipenem ( IMI ) .
	manualset3
177612	3	411014	13	NULL	NULL	0	NULL	liquid micro dilution technic	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimum inhibitory concentrations of the following antibiotics were performed by a liquid micro dilution technic : amoxicillin ( AMX ) , amoxicillin + clavulanic acid ( CL ) , 5 mg/l , ticarcillin ( TIC ) , piperacillin ( PIP ) , cefazolin ( CEZ ) , cefamandole ( CFM ) , cefoperazone ( CFP ) , cefotaxime ( CTX ) , cefotaxime + clavulanic acid 5 mg/l , cefotaxime + sulbactam ( SUL ) 5 mg/l , cefpirome ( CPI ) , ceftazidime ( CAZ ) , azthreonam ( AZT ) , latamoxef ( MOX ) , cefoxitin ( FOX ) , cefotetan ( CTT ) , temocillin ( TMO ) , imipenem ( IMI ) .
	manualset3
177613	4	411014	13	NULL	NULL	0	NULL	amoxicillin ( AMX )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimum inhibitory concentrations of the following antibiotics were performed by a liquid micro dilution technic : amoxicillin ( AMX ) , amoxicillin + clavulanic acid ( CL ) , 5 mg/l , ticarcillin ( TIC ) , piperacillin ( PIP ) , cefazolin ( CEZ ) , cefamandole ( CFM ) , cefoperazone ( CFP ) , cefotaxime ( CTX ) , cefotaxime + clavulanic acid 5 mg/l , cefotaxime + sulbactam ( SUL ) 5 mg/l , cefpirome ( CPI ) , ceftazidime ( CAZ ) , azthreonam ( AZT ) , latamoxef ( MOX ) , cefoxitin ( FOX ) , cefotetan ( CTT ) , temocillin ( TMO ) , imipenem ( IMI ) .
	manualset3
177614	5	411014	13	NULL	NULL	0	NULL	amoxicillin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimum inhibitory concentrations of the following antibiotics were performed by a liquid micro dilution technic : amoxicillin ( AMX ) , amoxicillin + clavulanic acid ( CL ) , 5 mg/l , ticarcillin ( TIC ) , piperacillin ( PIP ) , cefazolin ( CEZ ) , cefamandole ( CFM ) , cefoperazone ( CFP ) , cefotaxime ( CTX ) , cefotaxime + clavulanic acid 5 mg/l , cefotaxime + sulbactam ( SUL ) 5 mg/l , cefpirome ( CPI ) , ceftazidime ( CAZ ) , azthreonam ( AZT ) , latamoxef ( MOX ) , cefoxitin ( FOX ) , cefotetan ( CTT ) , temocillin ( TMO ) , imipenem ( IMI ) .
	manualset3
177615	6	411014	13	NULL	NULL	0	NULL	clavulanic acid 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimum inhibitory concentrations of the following antibiotics were performed by a liquid micro dilution technic : amoxicillin ( AMX ) , amoxicillin + clavulanic acid ( CL ) , 5 mg/l , ticarcillin ( TIC ) , piperacillin ( PIP ) , cefazolin ( CEZ ) , cefamandole ( CFM ) , cefoperazone ( CFP ) , cefotaxime ( CTX ) , cefotaxime + clavulanic acid 5 mg/l , cefotaxime + sulbactam ( SUL ) 5 mg/l , cefpirome ( CPI ) , ceftazidime ( CAZ ) , azthreonam ( AZT ) , latamoxef ( MOX ) , cefoxitin ( FOX ) , cefotetan ( CTT ) , temocillin ( TMO ) , imipenem ( IMI ) .
	manualset3
177616	7	411014	13	NULL	NULL	0	NULL	CL	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimum inhibitory concentrations of the following antibiotics were performed by a liquid micro dilution technic : amoxicillin ( AMX ) , amoxicillin + clavulanic acid ( CL ) , 5 mg/l , ticarcillin ( TIC ) , piperacillin ( PIP ) , cefazolin ( CEZ ) , cefamandole ( CFM ) , cefoperazone ( CFP ) , cefotaxime ( CTX ) , cefotaxime + clavulanic acid 5 mg/l , cefotaxime + sulbactam ( SUL ) 5 mg/l , cefpirome ( CPI ) , ceftazidime ( CAZ ) , azthreonam ( AZT ) , latamoxef ( MOX ) , cefoxitin ( FOX ) , cefotetan ( CTT ) , temocillin ( TMO ) , imipenem ( IMI ) .
	manualset3
177617	8	411014	13	NULL	NULL	0	NULL	5 mg/l	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimum inhibitory concentrations of the following antibiotics were performed by a liquid micro dilution technic : amoxicillin ( AMX ) , amoxicillin + clavulanic acid ( CL ) , 5 mg/l , ticarcillin ( TIC ) , piperacillin ( PIP ) , cefazolin ( CEZ ) , cefamandole ( CFM ) , cefoperazone ( CFP ) , cefotaxime ( CTX ) , cefotaxime + clavulanic acid 5 mg/l , cefotaxime + sulbactam ( SUL ) 5 mg/l , cefpirome ( CPI ) , ceftazidime ( CAZ ) , azthreonam ( AZT ) , latamoxef ( MOX ) , cefoxitin ( FOX ) , cefotetan ( CTT ) , temocillin ( TMO ) , imipenem ( IMI ) .
	manualset3
177618	9	411014	13	NULL	NULL	0	NULL	ticarcillin ( TIC )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimum inhibitory concentrations of the following antibiotics were performed by a liquid micro dilution technic : amoxicillin ( AMX ) , amoxicillin + clavulanic acid ( CL ) , 5 mg/l , ticarcillin ( TIC ) , piperacillin ( PIP ) , cefazolin ( CEZ ) , cefamandole ( CFM ) , cefoperazone ( CFP ) , cefotaxime ( CTX ) , cefotaxime + clavulanic acid 5 mg/l , cefotaxime + sulbactam ( SUL ) 5 mg/l , cefpirome ( CPI ) , ceftazidime ( CAZ ) , azthreonam ( AZT ) , latamoxef ( MOX ) , cefoxitin ( FOX ) , cefotetan ( CTT ) , temocillin ( TMO ) , imipenem ( IMI ) .
	manualset3
177619	10	411014	13	NULL	NULL	0	NULL	piperacillin ( PIP ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimum inhibitory concentrations of the following antibiotics were performed by a liquid micro dilution technic : amoxicillin ( AMX ) , amoxicillin + clavulanic acid ( CL ) , 5 mg/l , ticarcillin ( TIC ) , piperacillin ( PIP ) , cefazolin ( CEZ ) , cefamandole ( CFM ) , cefoperazone ( CFP ) , cefotaxime ( CTX ) , cefotaxime + clavulanic acid 5 mg/l , cefotaxime + sulbactam ( SUL ) 5 mg/l , cefpirome ( CPI ) , ceftazidime ( CAZ ) , azthreonam ( AZT ) , latamoxef ( MOX ) , cefoxitin ( FOX ) , cefotetan ( CTT ) , temocillin ( TMO ) , imipenem ( IMI ) .
	manualset3
177620	11	411014	13	NULL	NULL	0	NULL	cefazolin ( CEZ ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimum inhibitory concentrations of the following antibiotics were performed by a liquid micro dilution technic : amoxicillin ( AMX ) , amoxicillin + clavulanic acid ( CL ) , 5 mg/l , ticarcillin ( TIC ) , piperacillin ( PIP ) , cefazolin ( CEZ ) , cefamandole ( CFM ) , cefoperazone ( CFP ) , cefotaxime ( CTX ) , cefotaxime + clavulanic acid 5 mg/l , cefotaxime + sulbactam ( SUL ) 5 mg/l , cefpirome ( CPI ) , ceftazidime ( CAZ ) , azthreonam ( AZT ) , latamoxef ( MOX ) , cefoxitin ( FOX ) , cefotetan ( CTT ) , temocillin ( TMO ) , imipenem ( IMI ) .
	manualset3
177621	12	411014	13	NULL	NULL	0	NULL	cefamandole ( CFM ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimum inhibitory concentrations of the following antibiotics were performed by a liquid micro dilution technic : amoxicillin ( AMX ) , amoxicillin + clavulanic acid ( CL ) , 5 mg/l , ticarcillin ( TIC ) , piperacillin ( PIP ) , cefazolin ( CEZ ) , cefamandole ( CFM ) , cefoperazone ( CFP ) , cefotaxime ( CTX ) , cefotaxime + clavulanic acid 5 mg/l , cefotaxime + sulbactam ( SUL ) 5 mg/l , cefpirome ( CPI ) , ceftazidime ( CAZ ) , azthreonam ( AZT ) , latamoxef ( MOX ) , cefoxitin ( FOX ) , cefotetan ( CTT ) , temocillin ( TMO ) , imipenem ( IMI ) .
	manualset3
177622	13	411014	13	NULL	NULL	0	NULL	cefoperazone ( CFP ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimum inhibitory concentrations of the following antibiotics were performed by a liquid micro dilution technic : amoxicillin ( AMX ) , amoxicillin + clavulanic acid ( CL ) , 5 mg/l , ticarcillin ( TIC ) , piperacillin ( PIP ) , cefazolin ( CEZ ) , cefamandole ( CFM ) , cefoperazone ( CFP ) , cefotaxime ( CTX ) , cefotaxime + clavulanic acid 5 mg/l , cefotaxime + sulbactam ( SUL ) 5 mg/l , cefpirome ( CPI ) , ceftazidime ( CAZ ) , azthreonam ( AZT ) , latamoxef ( MOX ) , cefoxitin ( FOX ) , cefotetan ( CTT ) , temocillin ( TMO ) , imipenem ( IMI ) .
	manualset3
177623	14	411014	13	NULL	NULL	0	NULL	cefotaxime ( CTX )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimum inhibitory concentrations of the following antibiotics were performed by a liquid micro dilution technic : amoxicillin ( AMX ) , amoxicillin + clavulanic acid ( CL ) , 5 mg/l , ticarcillin ( TIC ) , piperacillin ( PIP ) , cefazolin ( CEZ ) , cefamandole ( CFM ) , cefoperazone ( CFP ) , cefotaxime ( CTX ) , cefotaxime + clavulanic acid 5 mg/l , cefotaxime + sulbactam ( SUL ) 5 mg/l , cefpirome ( CPI ) , ceftazidime ( CAZ ) , azthreonam ( AZT ) , latamoxef ( MOX ) , cefoxitin ( FOX ) , cefotetan ( CTT ) , temocillin ( TMO ) , imipenem ( IMI ) .
	manualset3
177624	15	411014	13	NULL	NULL	0	NULL	cefotaxime	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimum inhibitory concentrations of the following antibiotics were performed by a liquid micro dilution technic : amoxicillin ( AMX ) , amoxicillin + clavulanic acid ( CL ) , 5 mg/l , ticarcillin ( TIC ) , piperacillin ( PIP ) , cefazolin ( CEZ ) , cefamandole ( CFM ) , cefoperazone ( CFP ) , cefotaxime ( CTX ) , cefotaxime + clavulanic acid 5 mg/l , cefotaxime + sulbactam ( SUL ) 5 mg/l , cefpirome ( CPI ) , ceftazidime ( CAZ ) , azthreonam ( AZT ) , latamoxef ( MOX ) , cefoxitin ( FOX ) , cefotetan ( CTT ) , temocillin ( TMO ) , imipenem ( IMI ) .
	manualset3
177625	16	411014	13	NULL	NULL	0	NULL	clavulanic acid	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimum inhibitory concentrations of the following antibiotics were performed by a liquid micro dilution technic : amoxicillin ( AMX ) , amoxicillin + clavulanic acid ( CL ) , 5 mg/l , ticarcillin ( TIC ) , piperacillin ( PIP ) , cefazolin ( CEZ ) , cefamandole ( CFM ) , cefoperazone ( CFP ) , cefotaxime ( CTX ) , cefotaxime + clavulanic acid 5 mg/l , cefotaxime + sulbactam ( SUL ) 5 mg/l , cefpirome ( CPI ) , ceftazidime ( CAZ ) , azthreonam ( AZT ) , latamoxef ( MOX ) , cefoxitin ( FOX ) , cefotetan ( CTT ) , temocillin ( TMO ) , imipenem ( IMI ) .
	manualset3
177626	17	411014	13	NULL	NULL	0	NULL	5 mg/l 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimum inhibitory concentrations of the following antibiotics were performed by a liquid micro dilution technic : amoxicillin ( AMX ) , amoxicillin + clavulanic acid ( CL ) , 5 mg/l , ticarcillin ( TIC ) , piperacillin ( PIP ) , cefazolin ( CEZ ) , cefamandole ( CFM ) , cefoperazone ( CFP ) , cefotaxime ( CTX ) , cefotaxime + clavulanic acid 5 mg/l , cefotaxime + sulbactam ( SUL ) 5 mg/l , cefpirome ( CPI ) , ceftazidime ( CAZ ) , azthreonam ( AZT ) , latamoxef ( MOX ) , cefoxitin ( FOX ) , cefotetan ( CTT ) , temocillin ( TMO ) , imipenem ( IMI ) .
	manualset3
177627	18	411014	13	NULL	NULL	0	NULL	cefotaxime 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimum inhibitory concentrations of the following antibiotics were performed by a liquid micro dilution technic : amoxicillin ( AMX ) , amoxicillin + clavulanic acid ( CL ) , 5 mg/l , ticarcillin ( TIC ) , piperacillin ( PIP ) , cefazolin ( CEZ ) , cefamandole ( CFM ) , cefoperazone ( CFP ) , cefotaxime ( CTX ) , cefotaxime + clavulanic acid 5 mg/l , cefotaxime + sulbactam ( SUL ) 5 mg/l , cefpirome ( CPI ) , ceftazidime ( CAZ ) , azthreonam ( AZT ) , latamoxef ( MOX ) , cefoxitin ( FOX ) , cefotetan ( CTT ) , temocillin ( TMO ) , imipenem ( IMI ) .
	manualset3
177628	19	411014	13	NULL	NULL	0	NULL	sulbactam ( SUL )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimum inhibitory concentrations of the following antibiotics were performed by a liquid micro dilution technic : amoxicillin ( AMX ) , amoxicillin + clavulanic acid ( CL ) , 5 mg/l , ticarcillin ( TIC ) , piperacillin ( PIP ) , cefazolin ( CEZ ) , cefamandole ( CFM ) , cefoperazone ( CFP ) , cefotaxime ( CTX ) , cefotaxime + clavulanic acid 5 mg/l , cefotaxime + sulbactam ( SUL ) 5 mg/l , cefpirome ( CPI ) , ceftazidime ( CAZ ) , azthreonam ( AZT ) , latamoxef ( MOX ) , cefoxitin ( FOX ) , cefotetan ( CTT ) , temocillin ( TMO ) , imipenem ( IMI ) .
	manualset3
177629	20	411014	13	NULL	NULL	0	NULL	5 mg/l	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimum inhibitory concentrations of the following antibiotics were performed by a liquid micro dilution technic : amoxicillin ( AMX ) , amoxicillin + clavulanic acid ( CL ) , 5 mg/l , ticarcillin ( TIC ) , piperacillin ( PIP ) , cefazolin ( CEZ ) , cefamandole ( CFM ) , cefoperazone ( CFP ) , cefotaxime ( CTX ) , cefotaxime + clavulanic acid 5 mg/l , cefotaxime + sulbactam ( SUL ) 5 mg/l , cefpirome ( CPI ) , ceftazidime ( CAZ ) , azthreonam ( AZT ) , latamoxef ( MOX ) , cefoxitin ( FOX ) , cefotetan ( CTT ) , temocillin ( TMO ) , imipenem ( IMI ) .
	manualset3
177630	21	411014	13	NULL	NULL	0	NULL	cefpirome ( CPI )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimum inhibitory concentrations of the following antibiotics were performed by a liquid micro dilution technic : amoxicillin ( AMX ) , amoxicillin + clavulanic acid ( CL ) , 5 mg/l , ticarcillin ( TIC ) , piperacillin ( PIP ) , cefazolin ( CEZ ) , cefamandole ( CFM ) , cefoperazone ( CFP ) , cefotaxime ( CTX ) , cefotaxime + clavulanic acid 5 mg/l , cefotaxime + sulbactam ( SUL ) 5 mg/l , cefpirome ( CPI ) , ceftazidime ( CAZ ) , azthreonam ( AZT ) , latamoxef ( MOX ) , cefoxitin ( FOX ) , cefotetan ( CTT ) , temocillin ( TMO ) , imipenem ( IMI ) .
	manualset3
177631	22	411014	13	NULL	NULL	0	NULL	ceftazidime ( CAZ )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimum inhibitory concentrations of the following antibiotics were performed by a liquid micro dilution technic : amoxicillin ( AMX ) , amoxicillin + clavulanic acid ( CL ) , 5 mg/l , ticarcillin ( TIC ) , piperacillin ( PIP ) , cefazolin ( CEZ ) , cefamandole ( CFM ) , cefoperazone ( CFP ) , cefotaxime ( CTX ) , cefotaxime + clavulanic acid 5 mg/l , cefotaxime + sulbactam ( SUL ) 5 mg/l , cefpirome ( CPI ) , ceftazidime ( CAZ ) , azthreonam ( AZT ) , latamoxef ( MOX ) , cefoxitin ( FOX ) , cefotetan ( CTT ) , temocillin ( TMO ) , imipenem ( IMI ) .
	manualset3
177632	23	411014	13	NULL	NULL	0	NULL	azthreonam ( AZT )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimum inhibitory concentrations of the following antibiotics were performed by a liquid micro dilution technic : amoxicillin ( AMX ) , amoxicillin + clavulanic acid ( CL ) , 5 mg/l , ticarcillin ( TIC ) , piperacillin ( PIP ) , cefazolin ( CEZ ) , cefamandole ( CFM ) , cefoperazone ( CFP ) , cefotaxime ( CTX ) , cefotaxime + clavulanic acid 5 mg/l , cefotaxime + sulbactam ( SUL ) 5 mg/l , cefpirome ( CPI ) , ceftazidime ( CAZ ) , azthreonam ( AZT ) , latamoxef ( MOX ) , cefoxitin ( FOX ) , cefotetan ( CTT ) , temocillin ( TMO ) , imipenem ( IMI ) .
	manualset3
177633	24	411014	13	NULL	NULL	0	NULL	latamoxef ( MOX ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimum inhibitory concentrations of the following antibiotics were performed by a liquid micro dilution technic : amoxicillin ( AMX ) , amoxicillin + clavulanic acid ( CL ) , 5 mg/l , ticarcillin ( TIC ) , piperacillin ( PIP ) , cefazolin ( CEZ ) , cefamandole ( CFM ) , cefoperazone ( CFP ) , cefotaxime ( CTX ) , cefotaxime + clavulanic acid 5 mg/l , cefotaxime + sulbactam ( SUL ) 5 mg/l , cefpirome ( CPI ) , ceftazidime ( CAZ ) , azthreonam ( AZT ) , latamoxef ( MOX ) , cefoxitin ( FOX ) , cefotetan ( CTT ) , temocillin ( TMO ) , imipenem ( IMI ) .
	manualset3
177634	25	411014	13	NULL	NULL	0	NULL	cefoxitin ( FOX )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimum inhibitory concentrations of the following antibiotics were performed by a liquid micro dilution technic : amoxicillin ( AMX ) , amoxicillin + clavulanic acid ( CL ) , 5 mg/l , ticarcillin ( TIC ) , piperacillin ( PIP ) , cefazolin ( CEZ ) , cefamandole ( CFM ) , cefoperazone ( CFP ) , cefotaxime ( CTX ) , cefotaxime + clavulanic acid 5 mg/l , cefotaxime + sulbactam ( SUL ) 5 mg/l , cefpirome ( CPI ) , ceftazidime ( CAZ ) , azthreonam ( AZT ) , latamoxef ( MOX ) , cefoxitin ( FOX ) , cefotetan ( CTT ) , temocillin ( TMO ) , imipenem ( IMI ) .
	manualset3
177635	26	411014	13	NULL	NULL	0	NULL	cefotetan ( CTT )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimum inhibitory concentrations of the following antibiotics were performed by a liquid micro dilution technic : amoxicillin ( AMX ) , amoxicillin + clavulanic acid ( CL ) , 5 mg/l , ticarcillin ( TIC ) , piperacillin ( PIP ) , cefazolin ( CEZ ) , cefamandole ( CFM ) , cefoperazone ( CFP ) , cefotaxime ( CTX ) , cefotaxime + clavulanic acid 5 mg/l , cefotaxime + sulbactam ( SUL ) 5 mg/l , cefpirome ( CPI ) , ceftazidime ( CAZ ) , azthreonam ( AZT ) , latamoxef ( MOX ) , cefoxitin ( FOX ) , cefotetan ( CTT ) , temocillin ( TMO ) , imipenem ( IMI ) .
	manualset3
177636	27	411014	13	NULL	NULL	0	NULL	 temocillin ( TMO ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimum inhibitory concentrations of the following antibiotics were performed by a liquid micro dilution technic : amoxicillin ( AMX ) , amoxicillin + clavulanic acid ( CL ) , 5 mg/l , ticarcillin ( TIC ) , piperacillin ( PIP ) , cefazolin ( CEZ ) , cefamandole ( CFM ) , cefoperazone ( CFP ) , cefotaxime ( CTX ) , cefotaxime + clavulanic acid 5 mg/l , cefotaxime + sulbactam ( SUL ) 5 mg/l , cefpirome ( CPI ) , ceftazidime ( CAZ ) , azthreonam ( AZT ) , latamoxef ( MOX ) , cefoxitin ( FOX ) , cefotetan ( CTT ) , temocillin ( TMO ) , imipenem ( IMI ) .
	manualset3
177637	28	411014	13	NULL	NULL	0	NULL	imipenem ( IMI )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The minimum inhibitory concentrations of the following antibiotics were performed by a liquid micro dilution technic : amoxicillin ( AMX ) , amoxicillin + clavulanic acid ( CL ) , 5 mg/l , ticarcillin ( TIC ) , piperacillin ( PIP ) , cefazolin ( CEZ ) , cefamandole ( CFM ) , cefoperazone ( CFP ) , cefotaxime ( CTX ) , cefotaxime + clavulanic acid 5 mg/l , cefotaxime + sulbactam ( SUL ) 5 mg/l , cefpirome ( CPI ) , ceftazidime ( CAZ ) , azthreonam ( AZT ) , latamoxef ( MOX ) , cefoxitin ( FOX ) , cefotetan ( CTT ) , temocillin ( TMO ) , imipenem ( IMI ) .
	manualset3
177638	1	411015	13	NULL	NULL	0	NULL	mutagenic properties	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The miscoding and mutagenic properties of dG-C8-AAF and dG-C8-AF have been established ; these adducts are readily excised by DNA repair enzymes engaged in nucleotide excision repair .
	manualset3
177639	2	411015	13	NULL	NULL	0	NULL	dG-C8-AAF	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The miscoding and mutagenic properties of dG-C8-AAF and dG-C8-AF have been established ; these adducts are readily excised by DNA repair enzymes engaged in nucleotide excision repair .
	manualset3
177640	3	411015	13	NULL	NULL	0	NULL	dG-C8-AF	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The miscoding and mutagenic properties of dG-C8-AAF and dG-C8-AF have been established ; these adducts are readily excised by DNA repair enzymes engaged in nucleotide excision repair .
	manualset3
177641	4	411015	13	NULL	NULL	0	NULL	adducts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The miscoding and mutagenic properties of dG-C8-AAF and dG-C8-AF have been established ; these adducts are readily excised by DNA repair enzymes engaged in nucleotide excision repair .
	manualset3
177642	5	411015	13	NULL	NULL	0	NULL	DNA repair enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The miscoding and mutagenic properties of dG-C8-AAF and dG-C8-AF have been established ; these adducts are readily excised by DNA repair enzymes engaged in nucleotide excision repair .
	manualset3
177643	6	411015	13	NULL	NULL	0	NULL	nucleotide excision repair	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The miscoding and mutagenic properties of dG-C8-AAF and dG-C8-AF have been established ; these adducts are readily excised by DNA repair enzymes engaged in nucleotide excision repair .
	manualset3
177644	1	411016	13	NULL	NULL	0	NULL	mitochondrial DNA ( mtDNA ) 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitochondrial DNA ( mtDNA ) restriction fragment length polymorphisms presented here indicate that only P. canadensis-like mtDNA occurs in this population , suggesting that introgression likely occurred from hybrid males mating with P. canadensis females .
	manualset3
177645	2	411016	13	NULL	NULL	0	NULL	restriction fragment length polymorphisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitochondrial DNA ( mtDNA ) restriction fragment length polymorphisms presented here indicate that only P. canadensis-like mtDNA occurs in this population , suggesting that introgression likely occurred from hybrid males mating with P. canadensis females .
	manualset3
177646	3	411016	13	NULL	NULL	0	NULL	P. canadensis-like mtDNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitochondrial DNA ( mtDNA ) restriction fragment length polymorphisms presented here indicate that only P. canadensis-like mtDNA occurs in this population , suggesting that introgression likely occurred from hybrid males mating with P. canadensis females .
	manualset3
177647	4	411016	13	NULL	NULL	0	NULL	population	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitochondrial DNA ( mtDNA ) restriction fragment length polymorphisms presented here indicate that only P. canadensis-like mtDNA occurs in this population , suggesting that introgression likely occurred from hybrid males mating with P. canadensis females .
	manualset3
177648	5	411016	13	NULL	NULL	0	NULL	introgression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitochondrial DNA ( mtDNA ) restriction fragment length polymorphisms presented here indicate that only P. canadensis-like mtDNA occurs in this population , suggesting that introgression likely occurred from hybrid males mating with P. canadensis females .
	manualset3
177649	6	411016	13	NULL	NULL	0	NULL	hybrid males	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitochondrial DNA ( mtDNA ) restriction fragment length polymorphisms presented here indicate that only P. canadensis-like mtDNA occurs in this population , suggesting that introgression likely occurred from hybrid males mating with P. canadensis females .
	manualset3
177650	7	411016	13	NULL	NULL	0	NULL	P. canadensis females 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitochondrial DNA ( mtDNA ) restriction fragment length polymorphisms presented here indicate that only P. canadensis-like mtDNA occurs in this population , suggesting that introgression likely occurred from hybrid males mating with P. canadensis females .
	manualset3
177651	1	411017	13	NULL	NULL	0	NULL	mitochondrial apoptosis pathway	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitochondrial apoptosis pathway is controlled by the bcl-2 protein family .
	manualset3
177652	2	411017	13	NULL	NULL	0	NULL	bcl-2 protein family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitochondrial apoptosis pathway is controlled by the bcl-2 protein family .
	manualset3
177653	1	411018	13	NULL	NULL	0	NULL	mitochondrial carriers	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitochondrial carriers are a family of transport proteins that shuttle metabolites , nucleotides , and cofactors across the inner mitochondrial membrane .
	manualset3
177654	2	411018	13	NULL	NULL	0	NULL	family of transport proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitochondrial carriers are a family of transport proteins that shuttle metabolites , nucleotides , and cofactors across the inner mitochondrial membrane .
	manualset3
177655	3	411018	13	NULL	NULL	0	NULL	metabolites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitochondrial carriers are a family of transport proteins that shuttle metabolites , nucleotides , and cofactors across the inner mitochondrial membrane .
	manualset3
177656	4	411018	13	NULL	NULL	0	NULL	nucleotides	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitochondrial carriers are a family of transport proteins that shuttle metabolites , nucleotides , and cofactors across the inner mitochondrial membrane .
	manualset3
177657	5	411018	13	NULL	NULL	0	NULL	cofactors 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitochondrial carriers are a family of transport proteins that shuttle metabolites , nucleotides , and cofactors across the inner mitochondrial membrane .
	manualset3
177658	6	411018	13	NULL	NULL	0	NULL	inner mitochondrial membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitochondrial carriers are a family of transport proteins that shuttle metabolites , nucleotides , and cofactors across the inner mitochondrial membrane .
	manualset3
177681	1	411019	13	NULL	NULL	0	NULL	 mitochondrial cytochrome c N-terminal region 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitochondrial cytochrome c N-terminal region is critical for maturation by holocytochrome c synthase .
	manualset3
177682	2	411019	13	NULL	NULL	0	NULL	maturation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitochondrial cytochrome c N-terminal region is critical for maturation by holocytochrome c synthase .
	manualset3
177683	3	411019	13	NULL	NULL	0	NULL	holocytochrome c synthase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitochondrial cytochrome c N-terminal region is critical for maturation by holocytochrome c synthase .
	manualset3
177684	1	411020	13	NULL	NULL	0	NULL	mitogenic effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitogenic effect of 12-O-tetradecanoylphorbol-13-acetate on F3 cells is not mediated by endogenous prostaglandin formation .
	manualset3
177685	2	411020	13	NULL	NULL	0	NULL	12-O-tetradecanoylphorbol-13-acetate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitogenic effect of 12-O-tetradecanoylphorbol-13-acetate on F3 cells is not mediated by endogenous prostaglandin formation .
	manualset3
177686	3	411020	13	NULL	NULL	0	NULL	F3 cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitogenic effect of 12-O-tetradecanoylphorbol-13-acetate on F3 cells is not mediated by endogenous prostaglandin formation .
	manualset3
177687	4	411020	13	NULL	NULL	0	NULL	prostaglandin formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitogenic effect of 12-O-tetradecanoylphorbol-13-acetate on F3 cells is not mediated by endogenous prostaglandin formation .
	manualset3
177688	1	411021	13	NULL	NULL	0	NULL	mitotic index	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitotic index was low , the highest measured value was 4 mitotic figures per 10 high power fields corresponding to 2.78 mitotic figures per mm2 of epithelium in the microscope field .
	manualset3
177689	2	411021	13	NULL	NULL	0	NULL	value 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitotic index was low , the highest measured value was 4 mitotic figures per 10 high power fields corresponding to 2.78 mitotic figures per mm2 of epithelium in the microscope field .
	manualset3
177690	3	411021	13	NULL	NULL	0	NULL	4 mitotic figures per 10 high power fields 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitotic index was low , the highest measured value was 4 mitotic figures per 10 high power fields corresponding to 2.78 mitotic figures per mm2 of epithelium in the microscope field .
	manualset3
177691	4	411021	13	NULL	NULL	0	NULL	2.78 mitotic figures per mm2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitotic index was low , the highest measured value was 4 mitotic figures per 10 high power fields corresponding to 2.78 mitotic figures per mm2 of epithelium in the microscope field .
	manualset3
177692	5	411021	13	NULL	NULL	0	NULL	epithelium	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitotic index was low , the highest measured value was 4 mitotic figures per 10 high power fields corresponding to 2.78 mitotic figures per mm2 of epithelium in the microscope field .
	manualset3
177693	6	411021	13	NULL	NULL	0	NULL	microscope field	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitotic index was low , the highest measured value was 4 mitotic figures per 10 high power fields corresponding to 2.78 mitotic figures per mm2 of epithelium in the microscope field .
	manualset3
177694	1	411022	13	NULL	NULL	0	NULL	unique population 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A unique population of T lymphocytes , designated dendritic epidermal T cells ( DETC ) , homes to the murine epidermis during fetal development .
	manualset3
177695	2	411022	13	NULL	NULL	0	NULL	T lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A unique population of T lymphocytes , designated dendritic epidermal T cells ( DETC ) , homes to the murine epidermis during fetal development .
	manualset3
177696	3	411022	13	NULL	NULL	0	NULL	dendritic epidermal T cells ( DETC )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A unique population of T lymphocytes , designated dendritic epidermal T cells ( DETC ) , homes to the murine epidermis during fetal development .
	manualset3
177697	4	411022	13	NULL	NULL	0	NULL	homes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A unique population of T lymphocytes , designated dendritic epidermal T cells ( DETC ) , homes to the murine epidermis during fetal development .
	manualset3
177698	5	411022	13	NULL	NULL	0	NULL	murine epidermis	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	A unique population of T lymphocytes , designated dendritic epidermal T cells ( DETC ) , homes to the murine epidermis during fetal development .
	manualset3
177699	6	411022	13	NULL	NULL	0	NULL	fetal development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A unique population of T lymphocytes , designated dendritic epidermal T cells ( DETC ) , homes to the murine epidermis during fetal development .
	manualset3
177700	1	411023	13	NULL	NULL	0	NULL	mixtures	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The mixtures can be stored for short periods in ordinary containers in a dry place .
	manualset3
177701	2	411023	13	NULL	NULL	0	NULL	short periods	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The mixtures can be stored for short periods in ordinary containers in a dry place .
	manualset3
177702	3	411023	13	NULL	NULL	0	NULL	ordinary containers	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The mixtures can be stored for short periods in ordinary containers in a dry place .
	manualset3
177703	4	411023	13	NULL	NULL	0	NULL	dry place	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The mixtures can be stored for short periods in ordinary containers in a dry place .
	manualset3
177704	1	411024	13	NULL	NULL	0	NULL	 mmg 1 locus 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mmg 1 locus and the mt genome most probably interact and this nucleo-cytoplasmic interaction plays a role in determining the NA sensitivity of yeast cells .
	manualset3
177705	2	411024	13	NULL	NULL	0	NULL	mt genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The mmg 1 locus and the mt genome most probably interact and this nucleo-cytoplasmic interaction plays a role in determining the NA sensitivity of yeast cells .
	manualset3
177706	3	411024	13	NULL	NULL	0	NULL	nucleo-cytoplasmic interaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mmg 1 locus and the mt genome most probably interact and this nucleo-cytoplasmic interaction plays a role in determining the NA sensitivity of yeast cells .
	manualset3
177707	4	411024	13	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The mmg 1 locus and the mt genome most probably interact and this nucleo-cytoplasmic interaction plays a role in determining the NA sensitivity of yeast cells .
	manualset3
177708	5	411024	13	NULL	NULL	0	NULL	NA sensitivity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mmg 1 locus and the mt genome most probably interact and this nucleo-cytoplasmic interaction plays a role in determining the NA sensitivity of yeast cells .
	manualset3
177709	6	411024	13	NULL	NULL	0	NULL	yeast cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The mmg 1 locus and the mt genome most probably interact and this nucleo-cytoplasmic interaction plays a role in determining the NA sensitivity of yeast cells .
	manualset3
177710	1	411025	13	NULL	NULL	0	NULL	mobile phase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The mobile phase consisted of 750 ml of acetonitrile and 250 ml of 100 mmol/l phosphoric acid ( v/v ) to which sodium hydroxide had been added .
	manualset3
177711	2	411025	13	NULL	NULL	0	NULL	750 ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mobile phase consisted of 750 ml of acetonitrile and 250 ml of 100 mmol/l phosphoric acid ( v/v ) to which sodium hydroxide had been added .
	manualset3
177712	3	411025	13	NULL	NULL	0	NULL	acetonitrile	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The mobile phase consisted of 750 ml of acetonitrile and 250 ml of 100 mmol/l phosphoric acid ( v/v ) to which sodium hydroxide had been added .
	manualset3
177713	4	411025	13	NULL	NULL	0	NULL	250 ml of 100 mmol/l 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mobile phase consisted of 750 ml of acetonitrile and 250 ml of 100 mmol/l phosphoric acid ( v/v ) to which sodium hydroxide had been added .
	manualset3
177714	5	411025	13	NULL	NULL	0	NULL	phosphoric acid ( v/v )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The mobile phase consisted of 750 ml of acetonitrile and 250 ml of 100 mmol/l phosphoric acid ( v/v ) to which sodium hydroxide had been added .
	manualset3
177715	6	411025	13	NULL	NULL	0	NULL	sodium hydroxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The mobile phase consisted of 750 ml of acetonitrile and 250 ml of 100 mmol/l phosphoric acid ( v/v ) to which sodium hydroxide had been added .
	manualset3
177716	1	411026	13	NULL	NULL	0	NULL	mobility	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mobility of the nucleocapsid protein was unaffected by tunicamycin .
	manualset3
177717	2	411026	13	NULL	NULL	0	NULL	nucleocapsid protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mobility of the nucleocapsid protein was unaffected by tunicamycin .
	manualset3
177718	3	411026	13	NULL	NULL	0	NULL	tunicamycin 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The mobility of the nucleocapsid protein was unaffected by tunicamycin .
	manualset3
177729	1	411027	13	NULL	NULL	0	NULL	mobility 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mobility of these successful elements requires the protein encoded by open reading frame-1 ( ORF1p ) , which binds single-stranded RNA with high affinity and functions as a nucleic acid chaperone .
	manualset3
177731	2	411027	13	NULL	NULL	0	NULL	successful elements	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The mobility of these successful elements requires the protein encoded by open reading frame-1 ( ORF1p ) , which binds single-stranded RNA with high affinity and functions as a nucleic acid chaperone .
	manualset3
177733	3	411027	13	NULL	NULL	0	NULL	protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mobility of these successful elements requires the protein encoded by open reading frame-1 ( ORF1p ) , which binds single-stranded RNA with high affinity and functions as a nucleic acid chaperone .
	manualset3
177734	4	411027	13	NULL	NULL	0	NULL	open reading frame-1 ( ORF1p )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The mobility of these successful elements requires the protein encoded by open reading frame-1 ( ORF1p ) , which binds single-stranded RNA with high affinity and functions as a nucleic acid chaperone .
	manualset3
177735	5	411027	13	NULL	NULL	0	NULL	single-stranded RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The mobility of these successful elements requires the protein encoded by open reading frame-1 ( ORF1p ) , which binds single-stranded RNA with high affinity and functions as a nucleic acid chaperone .
	manualset3
177736	6	411027	13	NULL	NULL	0	NULL	high affinity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mobility of these successful elements requires the protein encoded by open reading frame-1 ( ORF1p ) , which binds single-stranded RNA with high affinity and functions as a nucleic acid chaperone .
	manualset3
177737	7	411027	13	NULL	NULL	0	NULL	functions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mobility of these successful elements requires the protein encoded by open reading frame-1 ( ORF1p ) , which binds single-stranded RNA with high affinity and functions as a nucleic acid chaperone .
	manualset3
177738	8	411027	13	NULL	NULL	0	NULL	nucleic acid chaperone	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The mobility of these successful elements requires the protein encoded by open reading frame-1 ( ORF1p ) , which binds single-stranded RNA with high affinity and functions as a nucleic acid chaperone .
	manualset3
177739	1	411028	13	NULL	NULL	0	NULL	mobilization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mobilization of glycogen was a specific trait resulting from a defect in mitochondrial function that could not be suppressed by mutations in the cAMP - and Pho85 protein kinase-dependent nutrient-sensing pathways , and by other mutations which favor glycogen synthesis .
	manualset3
177740	2	411028	13	NULL	NULL	0	NULL	glycogen	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The mobilization of glycogen was a specific trait resulting from a defect in mitochondrial function that could not be suppressed by mutations in the cAMP - and Pho85 protein kinase-dependent nutrient-sensing pathways , and by other mutations which favor glycogen synthesis .
	manualset3
177741	3	411028	13	NULL	NULL	0	NULL	specific trait	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mobilization of glycogen was a specific trait resulting from a defect in mitochondrial function that could not be suppressed by mutations in the cAMP - and Pho85 protein kinase-dependent nutrient-sensing pathways , and by other mutations which favor glycogen synthesis .
	manualset3
177742	4	411028	13	NULL	NULL	0	NULL	 defect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mobilization of glycogen was a specific trait resulting from a defect in mitochondrial function that could not be suppressed by mutations in the cAMP - and Pho85 protein kinase-dependent nutrient-sensing pathways , and by other mutations which favor glycogen synthesis .
	manualset3
177743	5	411028	13	NULL	NULL	0	NULL	mitochondrial function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mobilization of glycogen was a specific trait resulting from a defect in mitochondrial function that could not be suppressed by mutations in the cAMP - and Pho85 protein kinase-dependent nutrient-sensing pathways , and by other mutations which favor glycogen synthesis .
	manualset3
177756	6	411028	13	NULL	NULL	0	NULL	mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mobilization of glycogen was a specific trait resulting from a defect in mitochondrial function that could not be suppressed by mutations in the cAMP - and Pho85 protein kinase-dependent nutrient-sensing pathways , and by other mutations which favor glycogen synthesis .
	manualset3
177757	7	411028	13	NULL	NULL	0	NULL	cAMP - and Pho85 protein kinase-dependent nutrient-sensing pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mobilization of glycogen was a specific trait resulting from a defect in mitochondrial function that could not be suppressed by mutations in the cAMP - and Pho85 protein kinase-dependent nutrient-sensing pathways , and by other mutations which favor glycogen synthesis .
	manualset3
177758	8	411028	13	NULL	NULL	0	NULL	mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mobilization of glycogen was a specific trait resulting from a defect in mitochondrial function that could not be suppressed by mutations in the cAMP - and Pho85 protein kinase-dependent nutrient-sensing pathways , and by other mutations which favor glycogen synthesis .
	manualset3
177759	9	411028	13	NULL	NULL	0	NULL	glycogen synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mobilization of glycogen was a specific trait resulting from a defect in mitochondrial function that could not be suppressed by mutations in the cAMP - and Pho85 protein kinase-dependent nutrient-sensing pathways , and by other mutations which favor glycogen synthesis .
	manualset3
177760	1	411029	13	NULL	NULL	0	NULL	model 's responses	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The model 's responses to natural stimuli are illustrated , both for excerpts of recorded music from a large database utilized by tempo-estimation models , and sequences of taps from a bimanual tapping task .
	manualset3
177762	2	411029	13	NULL	NULL	0	NULL	natural stimuli 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The model 's responses to natural stimuli are illustrated , both for excerpts of recorded music from a large database utilized by tempo-estimation models , and sequences of taps from a bimanual tapping task .
	manualset3
177764	3	411029	13	NULL	NULL	0	NULL	excerpts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The model 's responses to natural stimuli are illustrated , both for excerpts of recorded music from a large database utilized by tempo-estimation models , and sequences of taps from a bimanual tapping task .
	manualset3
177766	4	411029	13	NULL	NULL	0	NULL	music	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The model 's responses to natural stimuli are illustrated , both for excerpts of recorded music from a large database utilized by tempo-estimation models , and sequences of taps from a bimanual tapping task .
	manualset3
177768	5	411029	13	NULL	NULL	0	NULL	large database 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The model 's responses to natural stimuli are illustrated , both for excerpts of recorded music from a large database utilized by tempo-estimation models , and sequences of taps from a bimanual tapping task .
	manualset3
177770	6	411029	13	NULL	NULL	0	NULL	tempo-estimation models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The model 's responses to natural stimuli are illustrated , both for excerpts of recorded music from a large database utilized by tempo-estimation models , and sequences of taps from a bimanual tapping task .
	manualset3
177773	7	411029	13	NULL	NULL	NULL	NULL	sequences 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The model 's responses to natural stimuli are illustrated , both for excerpts of recorded music from a large database utilized by tempo-estimation models , and sequences of taps from a bimanual tapping task .
	manualset3
177774	8	411029	13	NULL	NULL	0	NULL	taps 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The model 's responses to natural stimuli are illustrated , both for excerpts of recorded music from a large database utilized by tempo-estimation models , and sequences of taps from a bimanual tapping task .
	manualset3
177775	9	411029	13	NULL	NULL	0	NULL	bimanual tapping task	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The model 's responses to natural stimuli are illustrated , both for excerpts of recorded music from a large database utilized by tempo-estimation models , and sequences of taps from a bimanual tapping task .
	manualset3
177777	1	411030	13	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The model can be used to estimate the unknown efficiency parameters , such as pi ( extraction ) .
	manualset3
177778	2	411030	13	NULL	NULL	0	NULL	efficiency parameters	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The model can be used to estimate the unknown efficiency parameters , such as pi ( extraction ) .
	manualset3
177779	3	411030	13	NULL	NULL	0	NULL	pi ( extraction )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The model can be used to estimate the unknown efficiency parameters , such as pi ( extraction ) .
	manualset3
178011	1	411031	13	NULL	NULL	0	NULL	 procedure 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A useful procedure is to apply a lubricant during finishing of the cement .
	manualset3
178012	2	411031	13	NULL	NULL	0	NULL	lubricant 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A useful procedure is to apply a lubricant during finishing of the cement .
	manualset3
178013	3	411031	13	NULL	NULL	0	NULL	cement	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A useful procedure is to apply a lubricant during finishing of the cement .
	manualset3
178014	1	411032	13	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The model consisted of layers , filled with liquid , containing scattering particles , at different distances to the optics of the flowmeter .
	manualset3
178015	2	411032	13	NULL	NULL	0	NULL	layers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The model consisted of layers , filled with liquid , containing scattering particles , at different distances to the optics of the flowmeter .
	manualset3
178016	3	411032	13	NULL	NULL	0	NULL	liquid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The model consisted of layers , filled with liquid , containing scattering particles , at different distances to the optics of the flowmeter .
	manualset3
178017	4	411032	13	NULL	NULL	0	NULL	scattering particles	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The model consisted of layers , filled with liquid , containing scattering particles , at different distances to the optics of the flowmeter .
	manualset3
178018	5	411032	13	NULL	NULL	0	NULL	distances 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The model consisted of layers , filled with liquid , containing scattering particles , at different distances to the optics of the flowmeter .
	manualset3
178019	6	411032	13	NULL	NULL	0	NULL	 optics	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The model consisted of layers , filled with liquid , containing scattering particles , at different distances to the optics of the flowmeter .
	manualset3
178020	7	411032	13	NULL	NULL	0	NULL	flowmeter	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The model consisted of layers , filled with liquid , containing scattering particles , at different distances to the optics of the flowmeter .
	manualset3
178021	1	411033	13	NULL	NULL	0	NULL	model framework 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The model framework comprised a landscape generator , a potato late blight model that includes host and pathogen life cycles and fungicide management at the field scale , and an atmospheric dispersion model that calculates spore dispersal at the landscape scale .
	manualset3
178022	2	411033	13	NULL	NULL	0	NULL	landscape generator	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The model framework comprised a landscape generator , a potato late blight model that includes host and pathogen life cycles and fungicide management at the field scale , and an atmospheric dispersion model that calculates spore dispersal at the landscape scale .
	manualset3
178023	3	411033	13	NULL	NULL	0	NULL	potato late blight model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The model framework comprised a landscape generator , a potato late blight model that includes host and pathogen life cycles and fungicide management at the field scale , and an atmospheric dispersion model that calculates spore dispersal at the landscape scale .
	manualset3
178024	4	411033	13	NULL	NULL	0	NULL	host life cycles	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The model framework comprised a landscape generator , a potato late blight model that includes host and pathogen life cycles and fungicide management at the field scale , and an atmospheric dispersion model that calculates spore dispersal at the landscape scale .
	manualset3
178026	5	411033	13	NULL	NULL	0	NULL	pathogen life cycles	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The model framework comprised a landscape generator , a potato late blight model that includes host and pathogen life cycles and fungicide management at the field scale , and an atmospheric dispersion model that calculates spore dispersal at the landscape scale .
	manualset3
178027	6	411033	13	NULL	NULL	0	NULL	fungicide management 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The model framework comprised a landscape generator , a potato late blight model that includes host and pathogen life cycles and fungicide management at the field scale , and an atmospheric dispersion model that calculates spore dispersal at the landscape scale .
	manualset3
178028	7	411033	13	NULL	NULL	NULL	NULL	field scale	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The model framework comprised a landscape generator , a potato late blight model that includes host and pathogen life cycles and fungicide management at the field scale , and an atmospheric dispersion model that calculates spore dispersal at the landscape scale .
	manualset3
178029	8	411033	13	NULL	NULL	0	NULL	atmospheric dispersion model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The model framework comprised a landscape generator , a potato late blight model that includes host and pathogen life cycles and fungicide management at the field scale , and an atmospheric dispersion model that calculates spore dispersal at the landscape scale .
	manualset3
178030	9	411033	13	NULL	NULL	0	NULL	spore	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The model framework comprised a landscape generator , a potato late blight model that includes host and pathogen life cycles and fungicide management at the field scale , and an atmospheric dispersion model that calculates spore dispersal at the landscape scale .
	manualset3
178031	10	411033	13	NULL	NULL	0	NULL	dispersal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The model framework comprised a landscape generator , a potato late blight model that includes host and pathogen life cycles and fungicide management at the field scale , and an atmospheric dispersion model that calculates spore dispersal at the landscape scale .
	manualset3
178032	11	411033	13	NULL	NULL	NULL	NULL	landscape scale	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The model framework comprised a landscape generator , a potato late blight model that includes host and pathogen life cycles and fungicide management at the field scale , and an atmospheric dispersion model that calculates spore dispersal at the landscape scale .
	manualset3
178033	1	411034	13	NULL	NULL	0	NULL	model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The model implies that it is unnecessary to invoke an internal load or multiple regulatory mechanisms to explain regulation of V0 in smooth muscle .
	manualset3
178034	2	411034	13	NULL	NULL	0	NULL	 internal load	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The model implies that it is unnecessary to invoke an internal load or multiple regulatory mechanisms to explain regulation of V0 in smooth muscle .
	manualset3
178035	3	411034	13	NULL	NULL	0	NULL	regulatory mechanisms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The model implies that it is unnecessary to invoke an internal load or multiple regulatory mechanisms to explain regulation of V0 in smooth muscle .
	manualset3
178036	4	411034	13	NULL	NULL	0	NULL	regulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The model implies that it is unnecessary to invoke an internal load or multiple regulatory mechanisms to explain regulation of V0 in smooth muscle .
	manualset3
178037	5	411034	13	NULL	NULL	0	NULL	V0	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The model implies that it is unnecessary to invoke an internal load or multiple regulatory mechanisms to explain regulation of V0 in smooth muscle .
	manualset3
178038	6	411034	13	NULL	NULL	0	NULL	smooth muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The model implies that it is unnecessary to invoke an internal load or multiple regulatory mechanisms to explain regulation of V0 in smooth muscle .
	manualset3
178039	1	411035	13	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The model recognizes a single health benefit -- reduced head injuries -- and a single health cost-increased morbidity due to foregone exercise from reduced cycling .
	manualset3
178040	2	411035	13	NULL	NULL	0	NULL	single health benefit 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The model recognizes a single health benefit -- reduced head injuries -- and a single health cost-increased morbidity due to foregone exercise from reduced cycling .
	manualset3
178041	3	411035	13	NULL	NULL	0	NULL	 head injuries	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The model recognizes a single health benefit -- reduced head injuries -- and a single health cost-increased morbidity due to foregone exercise from reduced cycling .
	manualset3
178042	4	411035	13	NULL	NULL	0	NULL	health cost	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The model recognizes a single health benefit -- reduced head injuries -- and a single health cost-increased morbidity due to foregone exercise from reduced cycling .
	manualset3
178043	5	411035	13	NULL	NULL	0	NULL	 morbidity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The model recognizes a single health benefit -- reduced head injuries -- and a single health cost-increased morbidity due to foregone exercise from reduced cycling .
	manualset3
178044	6	411035	13	NULL	NULL	0	NULL	 exercise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The model recognizes a single health benefit -- reduced head injuries -- and a single health cost-increased morbidity due to foregone exercise from reduced cycling .
	manualset3
178045	1	411036	13	NULL	NULL	0	NULL	model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The model represents the local environment of a single blood vessel .
	manualset3
178046	2	411036	13	NULL	NULL	0	NULL	local environment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The model represents the local environment of a single blood vessel .
	manualset3
178047	3	411036	13	NULL	NULL	0	NULL	single blood vessel	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The model represents the local environment of a single blood vessel .
	manualset3
178048	1	411037	13	NULL	NULL	0	NULL	user 's guide	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A user 's guide to flexible cystoscopes .
	manualset3
178049	2	411037	13	NULL	NULL	0	NULL	flexible cystoscopes	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	A user 's guide to flexible cystoscopes .
	manualset3
178050	1	411038	13	NULL	NULL	0	NULL	model simulation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The model simulation also showed that roots behave as reversibly leaky cable in water uptake .
	manualset3
178051	2	411038	13	NULL	NULL	0	NULL	roots	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The model simulation also showed that roots behave as reversibly leaky cable in water uptake .
	manualset3
178052	3	411038	13	NULL	NULL	0	NULL	cable 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The model simulation also showed that roots behave as reversibly leaky cable in water uptake .
	manualset3
178053	4	411038	13	NULL	NULL	0	NULL	water uptake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The model simulation also showed that roots behave as reversibly leaky cable in water uptake .
	manualset3
178054	1	411039	13	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The model suggested that PEI loading dramatically reduced free circulation and increased nonspecific adhesion to the vasculature .
	manualset3
178055	2	411039	13	NULL	NULL	0	NULL	PEI loading	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The model suggested that PEI loading dramatically reduced free circulation and increased nonspecific adhesion to the vasculature .
	manualset3
178056	3	411039	13	NULL	NULL	0	NULL	 circulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The model suggested that PEI loading dramatically reduced free circulation and increased nonspecific adhesion to the vasculature .
	manualset3
178057	4	411039	13	NULL	NULL	0	NULL	adhesion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The model suggested that PEI loading dramatically reduced free circulation and increased nonspecific adhesion to the vasculature .
	manualset3
178058	5	411039	13	NULL	NULL	0	NULL	vasculature	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The model suggested that PEI loading dramatically reduced free circulation and increased nonspecific adhesion to the vasculature .
	manualset3
178059	1	411040	13	NULL	NULL	0	NULL	 model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The model takes into account the actual voltage used to control the liquid movement in electrowetting ( lower than the applied voltage ) , the amount of surfactant adsorbed at the decane/water interface , and the dipole moment of the surfactant molecules .
	manualset3
178060	2	411040	13	NULL	NULL	0	NULL	account	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The model takes into account the actual voltage used to control the liquid movement in electrowetting ( lower than the applied voltage ) , the amount of surfactant adsorbed at the decane/water interface , and the dipole moment of the surfactant molecules .
	manualset3
178061	3	411040	13	NULL	NULL	0	NULL	voltage	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The model takes into account the actual voltage used to control the liquid movement in electrowetting ( lower than the applied voltage ) , the amount of surfactant adsorbed at the decane/water interface , and the dipole moment of the surfactant molecules .
	manualset3
178062	4	411040	13	NULL	NULL	0	NULL	 liquid movement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The model takes into account the actual voltage used to control the liquid movement in electrowetting ( lower than the applied voltage ) , the amount of surfactant adsorbed at the decane/water interface , and the dipole moment of the surfactant molecules .
	manualset3
178063	5	411040	13	NULL	NULL	0	NULL	voltage	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The model takes into account the actual voltage used to control the liquid movement in electrowetting ( lower than the applied voltage ) , the amount of surfactant adsorbed at the decane/water interface , and the dipole moment of the surfactant molecules .
	manualset3
178064	6	411040	13	NULL	NULL	0	NULL	amount	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The model takes into account the actual voltage used to control the liquid movement in electrowetting ( lower than the applied voltage ) , the amount of surfactant adsorbed at the decane/water interface , and the dipole moment of the surfactant molecules .
	manualset3
178065	7	411040	13	NULL	NULL	0	NULL	surfactant	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The model takes into account the actual voltage used to control the liquid movement in electrowetting ( lower than the applied voltage ) , the amount of surfactant adsorbed at the decane/water interface , and the dipole moment of the surfactant molecules .
	manualset3
178066	8	411040	13	NULL	NULL	0	NULL	decane/water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The model takes into account the actual voltage used to control the liquid movement in electrowetting ( lower than the applied voltage ) , the amount of surfactant adsorbed at the decane/water interface , and the dipole moment of the surfactant molecules .
	manualset3
178067	9	411040	13	NULL	NULL	0	NULL	interface 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The model takes into account the actual voltage used to control the liquid movement in electrowetting ( lower than the applied voltage ) , the amount of surfactant adsorbed at the decane/water interface , and the dipole moment of the surfactant molecules .
	manualset3
178068	10	411040	13	NULL	NULL	0	NULL	dipole moment 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The model takes into account the actual voltage used to control the liquid movement in electrowetting ( lower than the applied voltage ) , the amount of surfactant adsorbed at the decane/water interface , and the dipole moment of the surfactant molecules .
	manualset3
178069	11	411040	13	NULL	NULL	0	NULL	surfactant molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The model takes into account the actual voltage used to control the liquid movement in electrowetting ( lower than the applied voltage ) , the amount of surfactant adsorbed at the decane/water interface , and the dipole moment of the surfactant molecules .
	manualset3
178070	1	411041	13	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The model was defined by replacing the ACL with a mesh or tape Dacron prosthesis in 16 Beagle dogs .
	manualset3
178071	2	411041	13	NULL	NULL	0	NULL	ACL 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The model was defined by replacing the ACL with a mesh or tape Dacron prosthesis in 16 Beagle dogs .
	manualset3
178072	3	411041	13	NULL	NULL	0	NULL	mesh	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The model was defined by replacing the ACL with a mesh or tape Dacron prosthesis in 16 Beagle dogs .
	manualset3
178073	4	411041	13	NULL	NULL	0	NULL	tape Dacron prosthesis	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The model was defined by replacing the ACL with a mesh or tape Dacron prosthesis in 16 Beagle dogs .
	manualset3
178074	5	411041	13	NULL	NULL	0	NULL	16 Beagle dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The model was defined by replacing the ACL with a mesh or tape Dacron prosthesis in 16 Beagle dogs .
	manualset3
178075	1	411042	13	NULL	NULL	0	NULL	model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The model with constant linear HOA blur predicts well the improvement in human optical quality between infant and adult .
	manualset3
178076	2	411042	13	NULL	NULL	0	NULL	linear HOA blur	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The model with constant linear HOA blur predicts well the improvement in human optical quality between infant and adult .
	manualset3
178077	3	411042	13	NULL	NULL	0	NULL	 improvement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The model with constant linear HOA blur predicts well the improvement in human optical quality between infant and adult .
	manualset3
178078	4	411042	13	NULL	NULL	0	NULL	human optical quality 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The model with constant linear HOA blur predicts well the improvement in human optical quality between infant and adult .
	manualset3
178079	5	411042	13	NULL	NULL	NULL	NULL	infant	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The model with constant linear HOA blur predicts well the improvement in human optical quality between infant and adult .
	manualset3
178080	6	411042	13	NULL	NULL	0	NULL	adult	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The model with constant linear HOA blur predicts well the improvement in human optical quality between infant and adult .
	manualset3
178081	1	411043	13	NULL	NULL	0	NULL	modification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The modification of screen diffusion batteries to incorporate multiple screens of differing mesh number , called graded screen arrays , have permitted improved size resolution below 10 nm such that the size distributions can now be determined down to molecular sized activities ( 0.5 nm ) .
	manualset3
178082	2	411043	13	NULL	NULL	0	NULL	screen diffusion batteries	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The modification of screen diffusion batteries to incorporate multiple screens of differing mesh number , called graded screen arrays , have permitted improved size resolution below 10 nm such that the size distributions can now be determined down to molecular sized activities ( 0.5 nm ) .
	manualset3
178083	3	411043	13	NULL	NULL	0	NULL	multiple screens 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The modification of screen diffusion batteries to incorporate multiple screens of differing mesh number , called graded screen arrays , have permitted improved size resolution below 10 nm such that the size distributions can now be determined down to molecular sized activities ( 0.5 nm ) .
	manualset3
178084	4	411043	13	NULL	NULL	0	NULL	mesh number	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The modification of screen diffusion batteries to incorporate multiple screens of differing mesh number , called graded screen arrays , have permitted improved size resolution below 10 nm such that the size distributions can now be determined down to molecular sized activities ( 0.5 nm ) .
	manualset3
178085	5	411043	13	NULL	NULL	0	NULL	screen arrays 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The modification of screen diffusion batteries to incorporate multiple screens of differing mesh number , called graded screen arrays , have permitted improved size resolution below 10 nm such that the size distributions can now be determined down to molecular sized activities ( 0.5 nm ) .
	manualset3
178086	6	411043	13	NULL	NULL	0	NULL	size resolution 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The modification of screen diffusion batteries to incorporate multiple screens of differing mesh number , called graded screen arrays , have permitted improved size resolution below 10 nm such that the size distributions can now be determined down to molecular sized activities ( 0.5 nm ) .
	manualset3
178087	7	411043	13	NULL	NULL	0	NULL	10 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The modification of screen diffusion batteries to incorporate multiple screens of differing mesh number , called graded screen arrays , have permitted improved size resolution below 10 nm such that the size distributions can now be determined down to molecular sized activities ( 0.5 nm ) .
	manualset3
178088	8	411043	13	NULL	NULL	0	NULL	size 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The modification of screen diffusion batteries to incorporate multiple screens of differing mesh number , called graded screen arrays , have permitted improved size resolution below 10 nm such that the size distributions can now be determined down to molecular sized activities ( 0.5 nm ) .
	manualset3
178089	9	411043	13	NULL	NULL	0	NULL	distributions 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The modification of screen diffusion batteries to incorporate multiple screens of differing mesh number , called graded screen arrays , have permitted improved size resolution below 10 nm such that the size distributions can now be determined down to molecular sized activities ( 0.5 nm ) .
	manualset3
178090	10	411043	13	NULL	NULL	0	NULL	activities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The modification of screen diffusion batteries to incorporate multiple screens of differing mesh number , called graded screen arrays , have permitted improved size resolution below 10 nm such that the size distributions can now be determined down to molecular sized activities ( 0.5 nm ) .
	manualset3
178091	11	411043	13	NULL	NULL	0	NULL	0.5 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The modification of screen diffusion batteries to incorporate multiple screens of differing mesh number , called graded screen arrays , have permitted improved size resolution below 10 nm such that the size distributions can now be determined down to molecular sized activities ( 0.5 nm ) .
	manualset3
178092	1	411044	13	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The modulating effect of bacterial volatiles on plant growth : current knowledge and future challenges .
	manualset3
178093	2	411044	13	NULL	NULL	0	NULL	bacterial volatiles	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The modulating effect of bacterial volatiles on plant growth : current knowledge and future challenges .
	manualset3
178094	3	411044	13	NULL	NULL	0	NULL	plant growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The modulating effect of bacterial volatiles on plant growth : current knowledge and future challenges .
	manualset3
178095	4	411044	13	NULL	NULL	0	NULL	current knowledge	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The modulating effect of bacterial volatiles on plant growth : current knowledge and future challenges .
	manualset3
178096	5	411044	13	NULL	NULL	0	NULL	future challenges	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The modulating effect of bacterial volatiles on plant growth : current knowledge and future challenges .
	manualset3
178097	1	411045	13	NULL	NULL	0	NULL	Clinical experience	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical experience with radiation synovectomy in the treatment of chronic synovitis of the knee joint -- long-term investigation ( author 's transl ) ) .
	manualset3
178098	2	411045	13	NULL	NULL	NULL	NULL	radiation synovectomy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Clinical experience with radiation synovectomy in the treatment of chronic synovitis of the knee joint -- long-term investigation ( author 's transl ) ) .
	manualset3
178099	3	411045	13	NULL	NULL	NULL	NULL	treatment 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Clinical experience with radiation synovectomy in the treatment of chronic synovitis of the knee joint -- long-term investigation ( author 's transl ) ) .
	manualset3
178100	4	411045	13	NULL	NULL	0	NULL	chronic synovitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical experience with radiation synovectomy in the treatment of chronic synovitis of the knee joint -- long-term investigation ( author 's transl ) ) .
	manualset3
178101	5	411045	13	NULL	NULL	0	NULL	knee joint	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical experience with radiation synovectomy in the treatment of chronic synovitis of the knee joint -- long-term investigation ( author 's transl ) ) .
	manualset3
178102	6	411045	13	NULL	NULL	0	NULL	long-term investigation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical experience with radiation synovectomy in the treatment of chronic synovitis of the knee joint -- long-term investigation ( author 's transl ) ) .
	manualset3
178103	7	411045	13	NULL	NULL	0	NULL	author 's transl	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical experience with radiation synovectomy in the treatment of chronic synovitis of the knee joint -- long-term investigation ( author 's transl ) ) .
	manualset3
178104	1	411046	13	NULL	NULL	0	NULL	valuation trial 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A valuation trial of the usefulness of fine needle aspiration biopsy in breast cancer diagnosis attempted .
	manualset3
178105	2	411046	13	NULL	NULL	0	NULL	usefulness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A valuation trial of the usefulness of fine needle aspiration biopsy in breast cancer diagnosis attempted .
	manualset3
178106	3	411046	13	NULL	NULL	0	NULL	fine needle aspiration biopsy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A valuation trial of the usefulness of fine needle aspiration biopsy in breast cancer diagnosis attempted .
	manualset3
178107	4	411046	13	NULL	NULL	NULL	NULL	breast cancer 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A valuation trial of the usefulness of fine needle aspiration biopsy in breast cancer diagnosis attempted .
	manualset3
178108	5	411046	13	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A valuation trial of the usefulness of fine needle aspiration biopsy in breast cancer diagnosis attempted .
	manualset3
178109	1	411047	13	NULL	NULL	0	NULL	 modulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The modulation by chlormethiazole of the GABAA-receptor complex in rat brain .
	manualset3
178110	2	411047	13	NULL	NULL	0	NULL	chlormethiazole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The modulation by chlormethiazole of the GABAA-receptor complex in rat brain .
	manualset3
178111	3	411047	13	NULL	NULL	0	NULL	GABAA-receptor complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The modulation by chlormethiazole of the GABAA-receptor complex in rat brain .
	manualset3
178112	4	411047	13	NULL	NULL	0	NULL	rat brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The modulation by chlormethiazole of the GABAA-receptor complex in rat brain .
	manualset3
178113	1	411048	13	NULL	NULL	0	NULL	modulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The modulation of the interaction by calcium ions makes it unique among the currently known binding mechanisms of proteinaceous alpha-amylase inhibitors .
	manualset3
178114	2	411048	13	NULL	NULL	0	NULL	 interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The modulation of the interaction by calcium ions makes it unique among the currently known binding mechanisms of proteinaceous alpha-amylase inhibitors .
	manualset3
178115	3	411048	13	NULL	NULL	0	NULL	calcium ions 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The modulation of the interaction by calcium ions makes it unique among the currently known binding mechanisms of proteinaceous alpha-amylase inhibitors .
	manualset3
178116	4	411048	13	NULL	NULL	0	NULL	mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The modulation of the interaction by calcium ions makes it unique among the currently known binding mechanisms of proteinaceous alpha-amylase inhibitors .
	manualset3
178117	5	411048	13	NULL	NULL	0	NULL	proteinaceous alpha-amylase inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The modulation of the interaction by calcium ions makes it unique among the currently known binding mechanisms of proteinaceous alpha-amylase inhibitors .
	manualset3
178118	1	411049	13	NULL	NULL	0	NULL	modulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The modulation was associated with transient increases in inositol phosphate synthesis and intracellular Ca2 + and with phosphorylation of the EGF receptor on serine and threonine .
	manualset3
178119	2	411049	13	NULL	NULL	0	NULL	increases	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The modulation was associated with transient increases in inositol phosphate synthesis and intracellular Ca2 + and with phosphorylation of the EGF receptor on serine and threonine .
	manualset3
178120	3	411049	13	NULL	NULL	0	NULL	inositol phosphate synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The modulation was associated with transient increases in inositol phosphate synthesis and intracellular Ca2 + and with phosphorylation of the EGF receptor on serine and threonine .
	manualset3
178121	4	411049	13	NULL	NULL	0	NULL	intracellular Ca2 + 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The modulation was associated with transient increases in inositol phosphate synthesis and intracellular Ca2 + and with phosphorylation of the EGF receptor on serine and threonine .
	manualset3
178122	5	411049	13	NULL	NULL	0	NULL	phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The modulation was associated with transient increases in inositol phosphate synthesis and intracellular Ca2 + and with phosphorylation of the EGF receptor on serine and threonine .
	manualset3
178123	6	411049	13	NULL	NULL	0	NULL	 EGF receptor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The modulation was associated with transient increases in inositol phosphate synthesis and intracellular Ca2 + and with phosphorylation of the EGF receptor on serine and threonine .
	manualset3
178124	7	411049	13	NULL	NULL	0	NULL	serine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The modulation was associated with transient increases in inositol phosphate synthesis and intracellular Ca2 + and with phosphorylation of the EGF receptor on serine and threonine .
	manualset3
178125	8	411049	13	NULL	NULL	0	NULL	threonine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The modulation was associated with transient increases in inositol phosphate synthesis and intracellular Ca2 + and with phosphorylation of the EGF receptor on serine and threonine .
	manualset3
178126	1	411050	13	NULL	NULL	0	NULL	mol-ecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The mol-ecule has an E configuration about the C = N bond , and an intra-molecular hydrogen bond involving the hydoxyl substituent on the naphthyl ring and the N ' atom of the hydrazide .
	manualset3
178127	2	411050	13	NULL	NULL	0	NULL	E configuration 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mol-ecule has an E configuration about the C = N bond , and an intra-molecular hydrogen bond involving the hydoxyl substituent on the naphthyl ring and the N ' atom of the hydrazide .
	manualset3
178128	3	411050	13	NULL	NULL	0	NULL	C = N bond	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mol-ecule has an E configuration about the C = N bond , and an intra-molecular hydrogen bond involving the hydoxyl substituent on the naphthyl ring and the N ' atom of the hydrazide .
	manualset3
178129	4	411050	13	NULL	NULL	0	NULL	intra-molecular hydrogen bond	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mol-ecule has an E configuration about the C = N bond , and an intra-molecular hydrogen bond involving the hydoxyl substituent on the naphthyl ring and the N ' atom of the hydrazide .
	manualset3
178130	5	411050	13	NULL	NULL	0	NULL	hydoxyl substituent 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mol-ecule has an E configuration about the C = N bond , and an intra-molecular hydrogen bond involving the hydoxyl substituent on the naphthyl ring and the N ' atom of the hydrazide .
	manualset3
178131	6	411050	13	NULL	NULL	0	NULL	naphthyl ring	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The mol-ecule has an E configuration about the C = N bond , and an intra-molecular hydrogen bond involving the hydoxyl substituent on the naphthyl ring and the N ' atom of the hydrazide .
	manualset3
178132	7	411050	13	NULL	NULL	0	NULL	N ' atom	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The mol-ecule has an E configuration about the C = N bond , and an intra-molecular hydrogen bond involving the hydoxyl substituent on the naphthyl ring and the N ' atom of the hydrazide .
	manualset3
178133	8	411050	13	NULL	NULL	0	NULL	hydrazide 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The mol-ecule has an E configuration about the C = N bond , and an intra-molecular hydrogen bond involving the hydoxyl substituent on the naphthyl ring and the N ' atom of the hydrazide .
	manualset3
178134	1	411051	13	NULL	NULL	0	NULL	molecular identities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular and immunological identities between human and canine NC1 domains suggest that NC1 may be critical for the EBA development .
	manualset3
178135	2	411051	13	NULL	NULL	0	NULL	immunological identities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular and immunological identities between human and canine NC1 domains suggest that NC1 may be critical for the EBA development .
	manualset3
178136	3	411051	13	NULL	NULL	0	NULL	human NC1 domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular and immunological identities between human and canine NC1 domains suggest that NC1 may be critical for the EBA development .
	manualset3
178137	4	411051	13	NULL	NULL	0	NULL	canine NC1 domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular and immunological identities between human and canine NC1 domains suggest that NC1 may be critical for the EBA development .
	manualset3
178138	5	411051	13	NULL	NULL	0	NULL	NC1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular and immunological identities between human and canine NC1 domains suggest that NC1 may be critical for the EBA development .
	manualset3
178139	6	411051	13	NULL	NULL	0	NULL	EBA development 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular and immunological identities between human and canine NC1 domains suggest that NC1 may be critical for the EBA development .
	manualset3
178140	1	411052	13	NULL	NULL	0	NULL	 vapor-catalyzed surface immobilization scheme	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A vapor-catalyzed , isocyanate-mediated surface immobilization scheme is used to attach bioactive small molecules , natural products and small molecules derived from diversity-oriented synthesis pathways .
	manualset3
178141	2	411052	13	NULL	NULL	0	NULL	isocyanate-mediated surface immobilization scheme	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A vapor-catalyzed , isocyanate-mediated surface immobilization scheme is used to attach bioactive small molecules , natural products and small molecules derived from diversity-oriented synthesis pathways .
	manualset3
178142	3	411052	13	NULL	NULL	0	NULL	small molecules	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A vapor-catalyzed , isocyanate-mediated surface immobilization scheme is used to attach bioactive small molecules , natural products and small molecules derived from diversity-oriented synthesis pathways .
	manualset3
178143	4	411052	13	NULL	NULL	0	NULL	 natural products 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A vapor-catalyzed , isocyanate-mediated surface immobilization scheme is used to attach bioactive small molecules , natural products and small molecules derived from diversity-oriented synthesis pathways .
	manualset3
178144	5	411052	13	NULL	NULL	0	NULL	small molecules 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A vapor-catalyzed , isocyanate-mediated surface immobilization scheme is used to attach bioactive small molecules , natural products and small molecules derived from diversity-oriented synthesis pathways .
	manualset3
178145	6	411052	13	NULL	NULL	0	NULL	diversity-oriented synthesis pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A vapor-catalyzed , isocyanate-mediated surface immobilization scheme is used to attach bioactive small molecules , natural products and small molecules derived from diversity-oriented synthesis pathways .
	manualset3
178146	1	411053	13	NULL	NULL	0	NULL	molecular architecture 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular architecture of hARH3 constitutes the archetype of an all-alpha-helical protein fold and provides insights into the reversibility of protein ADP-ribosylation .
	manualset3
178147	2	411053	13	NULL	NULL	0	NULL	hARH3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular architecture of hARH3 constitutes the archetype of an all-alpha-helical protein fold and provides insights into the reversibility of protein ADP-ribosylation .
	manualset3
178148	3	411053	13	NULL	NULL	0	NULL	archetype	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular architecture of hARH3 constitutes the archetype of an all-alpha-helical protein fold and provides insights into the reversibility of protein ADP-ribosylation .
	manualset3
178149	4	411053	13	NULL	NULL	0	NULL	 all-alpha-helical protein fold 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular architecture of hARH3 constitutes the archetype of an all-alpha-helical protein fold and provides insights into the reversibility of protein ADP-ribosylation .
	manualset3
178150	5	411053	13	NULL	NULL	0	NULL	insights	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular architecture of hARH3 constitutes the archetype of an all-alpha-helical protein fold and provides insights into the reversibility of protein ADP-ribosylation .
	manualset3
178151	6	411053	13	NULL	NULL	0	NULL	reversibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular architecture of hARH3 constitutes the archetype of an all-alpha-helical protein fold and provides insights into the reversibility of protein ADP-ribosylation .
	manualset3
178152	7	411053	13	NULL	NULL	0	NULL	protein ADP-ribosylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular architecture of hARH3 constitutes the archetype of an all-alpha-helical protein fold and provides insights into the reversibility of protein ADP-ribosylation .
	manualset3
178153	1	411054	13	NULL	NULL	0	NULL	molecular basis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular basis for the extreme virulence of SARS-CoV remains elusive .
	manualset3
178154	2	411054	13	NULL	NULL	0	NULL	virulence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular basis for the extreme virulence of SARS-CoV remains elusive .
	manualset3
178155	3	411054	13	NULL	NULL	0	NULL	SARS-CoV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular basis for the extreme virulence of SARS-CoV remains elusive .
	manualset3
178156	1	411055	13	NULL	NULL	0	NULL	molecular basis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular basis of the observed species differences in response to PPs is unclear at present , but recent data support a quantitative hypothesis wherein PPARalpha expression levels are sufficient in humans to mediate hypolipidemia , but too low for transcriptional regulation of the full battery of genes associated with the adverse effects seen in rodents such as peroxisome proliferation , liver enlargement and tumors .
	manualset3
178157	2	411055	13	NULL	NULL	0	NULL	species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular basis of the observed species differences in response to PPs is unclear at present , but recent data support a quantitative hypothesis wherein PPARalpha expression levels are sufficient in humans to mediate hypolipidemia , but too low for transcriptional regulation of the full battery of genes associated with the adverse effects seen in rodents such as peroxisome proliferation , liver enlargement and tumors .
	manualset3
178158	3	411055	13	NULL	NULL	0	NULL	differences	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular basis of the observed species differences in response to PPs is unclear at present , but recent data support a quantitative hypothesis wherein PPARalpha expression levels are sufficient in humans to mediate hypolipidemia , but too low for transcriptional regulation of the full battery of genes associated with the adverse effects seen in rodents such as peroxisome proliferation , liver enlargement and tumors .
	manualset3
178159	4	411055	13	NULL	NULL	0	NULL	response	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular basis of the observed species differences in response to PPs is unclear at present , but recent data support a quantitative hypothesis wherein PPARalpha expression levels are sufficient in humans to mediate hypolipidemia , but too low for transcriptional regulation of the full battery of genes associated with the adverse effects seen in rodents such as peroxisome proliferation , liver enlargement and tumors .
	manualset3
178160	5	411055	13	NULL	NULL	0	NULL	PPs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular basis of the observed species differences in response to PPs is unclear at present , but recent data support a quantitative hypothesis wherein PPARalpha expression levels are sufficient in humans to mediate hypolipidemia , but too low for transcriptional regulation of the full battery of genes associated with the adverse effects seen in rodents such as peroxisome proliferation , liver enlargement and tumors .
	manualset3
178161	6	411055	13	NULL	NULL	0	NULL	 data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular basis of the observed species differences in response to PPs is unclear at present , but recent data support a quantitative hypothesis wherein PPARalpha expression levels are sufficient in humans to mediate hypolipidemia , but too low for transcriptional regulation of the full battery of genes associated with the adverse effects seen in rodents such as peroxisome proliferation , liver enlargement and tumors .
	manualset3
178162	7	411055	13	NULL	NULL	0	NULL	quantitative hypothesis 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular basis of the observed species differences in response to PPs is unclear at present , but recent data support a quantitative hypothesis wherein PPARalpha expression levels are sufficient in humans to mediate hypolipidemia , but too low for transcriptional regulation of the full battery of genes associated with the adverse effects seen in rodents such as peroxisome proliferation , liver enlargement and tumors .
	manualset3
178163	8	411055	13	NULL	NULL	0	NULL	PPARalpha expression levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular basis of the observed species differences in response to PPs is unclear at present , but recent data support a quantitative hypothesis wherein PPARalpha expression levels are sufficient in humans to mediate hypolipidemia , but too low for transcriptional regulation of the full battery of genes associated with the adverse effects seen in rodents such as peroxisome proliferation , liver enlargement and tumors .
	manualset3
178164	9	411055	13	NULL	NULL	0	NULL	humans	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular basis of the observed species differences in response to PPs is unclear at present , but recent data support a quantitative hypothesis wherein PPARalpha expression levels are sufficient in humans to mediate hypolipidemia , but too low for transcriptional regulation of the full battery of genes associated with the adverse effects seen in rodents such as peroxisome proliferation , liver enlargement and tumors .
	manualset3
178165	10	411055	13	NULL	NULL	0	NULL	 hypolipidemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular basis of the observed species differences in response to PPs is unclear at present , but recent data support a quantitative hypothesis wherein PPARalpha expression levels are sufficient in humans to mediate hypolipidemia , but too low for transcriptional regulation of the full battery of genes associated with the adverse effects seen in rodents such as peroxisome proliferation , liver enlargement and tumors .
	manualset3
178166	11	411055	13	NULL	NULL	0	NULL	transcriptional regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular basis of the observed species differences in response to PPs is unclear at present , but recent data support a quantitative hypothesis wherein PPARalpha expression levels are sufficient in humans to mediate hypolipidemia , but too low for transcriptional regulation of the full battery of genes associated with the adverse effects seen in rodents such as peroxisome proliferation , liver enlargement and tumors .
	manualset3
178167	12	411055	13	NULL	NULL	0	NULL	full battery of genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular basis of the observed species differences in response to PPs is unclear at present , but recent data support a quantitative hypothesis wherein PPARalpha expression levels are sufficient in humans to mediate hypolipidemia , but too low for transcriptional regulation of the full battery of genes associated with the adverse effects seen in rodents such as peroxisome proliferation , liver enlargement and tumors .
	manualset3
178168	13	411055	13	NULL	NULL	0	NULL	adverse effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular basis of the observed species differences in response to PPs is unclear at present , but recent data support a quantitative hypothesis wherein PPARalpha expression levels are sufficient in humans to mediate hypolipidemia , but too low for transcriptional regulation of the full battery of genes associated with the adverse effects seen in rodents such as peroxisome proliferation , liver enlargement and tumors .
	manualset3
178169	14	411055	13	NULL	NULL	0	NULL	rodents 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular basis of the observed species differences in response to PPs is unclear at present , but recent data support a quantitative hypothesis wherein PPARalpha expression levels are sufficient in humans to mediate hypolipidemia , but too low for transcriptional regulation of the full battery of genes associated with the adverse effects seen in rodents such as peroxisome proliferation , liver enlargement and tumors .
	manualset3
178170	15	411055	13	NULL	NULL	0	NULL	peroxisome proliferation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular basis of the observed species differences in response to PPs is unclear at present , but recent data support a quantitative hypothesis wherein PPARalpha expression levels are sufficient in humans to mediate hypolipidemia , but too low for transcriptional regulation of the full battery of genes associated with the adverse effects seen in rodents such as peroxisome proliferation , liver enlargement and tumors .
	manualset3
178171	16	411055	13	NULL	NULL	0	NULL	liver enlargement 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular basis of the observed species differences in response to PPs is unclear at present , but recent data support a quantitative hypothesis wherein PPARalpha expression levels are sufficient in humans to mediate hypolipidemia , but too low for transcriptional regulation of the full battery of genes associated with the adverse effects seen in rodents such as peroxisome proliferation , liver enlargement and tumors .
	manualset3
178172	17	411055	13	NULL	NULL	0	NULL	tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular basis of the observed species differences in response to PPs is unclear at present , but recent data support a quantitative hypothesis wherein PPARalpha expression levels are sufficient in humans to mediate hypolipidemia , but too low for transcriptional regulation of the full battery of genes associated with the adverse effects seen in rodents such as peroxisome proliferation , liver enlargement and tumors .
	manualset3
178173	1	411056	13	NULL	NULL	0	NULL	molecular masses of III	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular masses of III , IV , VII and VIII were found to be the same i.e. , 387 , while those of XIV and XV were 389 and 403 , respectively .
	manualset3
178174	2	411056	13	NULL	NULL	0	NULL	molecular masses of IV	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular masses of III , IV , VII and VIII were found to be the same i.e. , 387 , while those of XIV and XV were 389 and 403 , respectively .
	manualset3
178175	3	411056	13	NULL	NULL	0	NULL	molecular masses of VII	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular masses of III , IV , VII and VIII were found to be the same i.e. , 387 , while those of XIV and XV were 389 and 403 , respectively .
	manualset3
178176	4	411056	13	NULL	NULL	NULL	NULL	molecular masses of VIII	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The molecular masses of III , IV , VII and VIII were found to be the same i.e. , 387 , while those of XIV and XV were 389 and 403 , respectively .
	manualset3
178177	5	411056	13	NULL	NULL	0	NULL	 387	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular masses of III , IV , VII and VIII were found to be the same i.e. , 387 , while those of XIV and XV were 389 and 403 , respectively .
	manualset3
178178	6	411056	13	NULL	NULL	NULL	NULL	molecular masses of XIV	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The molecular masses of III , IV , VII and VIII were found to be the same i.e. , 387 , while those of XIV and XV were 389 and 403 , respectively .
	manualset3
178179	7	411056	13	NULL	NULL	NULL	NULL	molecular masses of XV	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The molecular masses of III , IV , VII and VIII were found to be the same i.e. , 387 , while those of XIV and XV were 389 and 403 , respectively .
	manualset3
178180	8	411056	13	NULL	NULL	0	NULL	389 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular masses of III , IV , VII and VIII were found to be the same i.e. , 387 , while those of XIV and XV were 389 and 403 , respectively .
	manualset3
178181	9	411056	13	NULL	NULL	0	NULL	403	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular masses of III , IV , VII and VIII were found to be the same i.e. , 387 , while those of XIV and XV were 389 and 403 , respectively .
	manualset3
178182	1	411057	13	NULL	NULL	0	NULL	molecular masses	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular masses of the glycoforms ranged from 95 to 135 kDa , but after deglycosylation , a single 68 kDa band was obtained .
	manualset3
178183	2	411057	13	NULL	NULL	0	NULL	glycoforms	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular masses of the glycoforms ranged from 95 to 135 kDa , but after deglycosylation , a single 68 kDa band was obtained .
	manualset3
178184	3	411057	13	NULL	NULL	0	NULL	95 to 135 kDa	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular masses of the glycoforms ranged from 95 to 135 kDa , but after deglycosylation , a single 68 kDa band was obtained .
	manualset3
178185	4	411057	13	NULL	NULL	0	NULL	deglycosylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular masses of the glycoforms ranged from 95 to 135 kDa , but after deglycosylation , a single 68 kDa band was obtained .
	manualset3
178186	5	411057	13	NULL	NULL	0	NULL	68 kDa band 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular masses of the glycoforms ranged from 95 to 135 kDa , but after deglycosylation , a single 68 kDa band was obtained .
	manualset3
178187	1	411058	13	NULL	NULL	0	NULL	molecular mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular mechanism underlying the bioluminescence reaction has remained unresolved , because the luciferase could not be identified or isolated .
	manualset3
178188	2	411058	13	NULL	NULL	0	NULL	bioluminescence reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular mechanism underlying the bioluminescence reaction has remained unresolved , because the luciferase could not be identified or isolated .
	manualset3
178189	3	411058	13	NULL	NULL	0	NULL	luciferase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular mechanism underlying the bioluminescence reaction has remained unresolved , because the luciferase could not be identified or isolated .
	manualset3
178190	1	411059	13	NULL	NULL	0	NULL	molecular mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular mechanisms of these dynamic Th cell responses and their impact on APC biology remain to be elucidated .
	manualset3
178191	2	411059	13	NULL	NULL	0	NULL	dynamic Th cell responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular mechanisms of these dynamic Th cell responses and their impact on APC biology remain to be elucidated .
	manualset3
178192	3	411059	13	NULL	NULL	0	NULL	impact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular mechanisms of these dynamic Th cell responses and their impact on APC biology remain to be elucidated .
	manualset3
178193	4	411059	13	NULL	NULL	0	NULL	APC biology	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular mechanisms of these dynamic Th cell responses and their impact on APC biology remain to be elucidated .
	manualset3
178194	1	411060	13	NULL	NULL	0	NULL	molecular phenotype	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular phenotype was revealed when troponin was dephosphorylated ; Ca ( 2 + ) - sensitivity of E361G-containing thin filaments was now lower than NTG ( EC ( 50 ) E361G ( dPTn ) / NTG ( dPTn ) = 2.15 + / -0.09 ) .
	manualset3
178195	2	411060	13	NULL	NULL	0	NULL	 troponin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular phenotype was revealed when troponin was dephosphorylated ; Ca ( 2 + ) - sensitivity of E361G-containing thin filaments was now lower than NTG ( EC ( 50 ) E361G ( dPTn ) / NTG ( dPTn ) = 2.15 + / -0.09 ) .
	manualset3
178196	3	411060	13	NULL	NULL	0	NULL	Ca ( 2 + ) - sensitivity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular phenotype was revealed when troponin was dephosphorylated ; Ca ( 2 + ) - sensitivity of E361G-containing thin filaments was now lower than NTG ( EC ( 50 ) E361G ( dPTn ) / NTG ( dPTn ) = 2.15 + / -0.09 ) .
	manualset3
178248	4	411060	13	NULL	NULL	0	NULL	E361G-containing thin filaments	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular phenotype was revealed when troponin was dephosphorylated ; Ca ( 2 + ) - sensitivity of E361G-containing thin filaments was now lower than NTG ( EC ( 50 ) E361G ( dPTn ) / NTG ( dPTn ) = 2.15 + / -0.09 ) .
	manualset3
178249	5	411060	13	NULL	NULL	0	NULL	NTG ( EC ( 50 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular phenotype was revealed when troponin was dephosphorylated ; Ca ( 2 + ) - sensitivity of E361G-containing thin filaments was now lower than NTG ( EC ( 50 ) E361G ( dPTn ) / NTG ( dPTn ) = 2.15 + / -0.09 ) .
	manualset3
178250	6	411060	13	NULL	NULL	0	NULL	E361G ( dPTn ) / NTG ( dPTn ) = 2.15 + / -0.09	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular phenotype was revealed when troponin was dephosphorylated ; Ca ( 2 + ) - sensitivity of E361G-containing thin filaments was now lower than NTG ( EC ( 50 ) E361G ( dPTn ) / NTG ( dPTn ) = 2.15 + / -0.09 ) .
	manualset3
178251	1	411061	13	NULL	NULL	0	NULL	molecular weight 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weight , isoelectric point , and N-terminal sequence of the purified peptide were determined .
	manualset3
178252	2	411061	13	NULL	NULL	0	NULL	isoelectric point 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weight , isoelectric point , and N-terminal sequence of the purified peptide were determined .
	manualset3
178253	3	411061	13	NULL	NULL	0	NULL	 N-terminal sequence 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weight , isoelectric point , and N-terminal sequence of the purified peptide were determined .
	manualset3
178254	4	411061	13	NULL	NULL	0	NULL	 peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weight , isoelectric point , and N-terminal sequence of the purified peptide were determined .
	manualset3
178255	1	411062	13	NULL	NULL	0	NULL	molecular weight	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weight and the isoelectric point of the activated prorenin were 40 , 000 and pH 4.9 .
	manualset3
178256	2	411062	13	NULL	NULL	0	NULL	isoelectric point	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weight and the isoelectric point of the activated prorenin were 40 , 000 and pH 4.9 .
	manualset3
178257	3	411062	13	NULL	NULL	0	NULL	prorenin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weight and the isoelectric point of the activated prorenin were 40 , 000 and pH 4.9 .
	manualset3
178258	4	411062	13	NULL	NULL	0	NULL	40 , 000	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weight and the isoelectric point of the activated prorenin were 40 , 000 and pH 4.9 .
	manualset3
178259	5	411062	13	NULL	NULL	0	NULL	pH 4.9	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weight and the isoelectric point of the activated prorenin were 40 , 000 and pH 4.9 .
	manualset3
178260	1	411063	13	NULL	NULL	0	NULL	variable degree 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A variable degree of coronary sinus thrombus was present in 18 dogs without clinical sequelae .
	manualset3
178261	2	411063	13	NULL	NULL	0	NULL	coronary sinus thrombus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A variable degree of coronary sinus thrombus was present in 18 dogs without clinical sequelae .
	manualset3
178262	3	411063	13	NULL	NULL	0	NULL	18 dogs 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A variable degree of coronary sinus thrombus was present in 18 dogs without clinical sequelae .
	manualset3
178263	4	411063	13	NULL	NULL	0	NULL	clinical sequelae 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A variable degree of coronary sinus thrombus was present in 18 dogs without clinical sequelae .
	manualset3
178264	1	411064	13	NULL	NULL	0	NULL	molecular weight 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weight of methyltransferase , calculated from the predicted amino acid sequence , was 21 , 700 .
	manualset3
178265	2	411064	13	NULL	NULL	0	NULL	methyltransferase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weight of methyltransferase , calculated from the predicted amino acid sequence , was 21 , 700 .
	manualset3
178266	3	411064	13	NULL	NULL	0	NULL	amino acid sequence	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weight of methyltransferase , calculated from the predicted amino acid sequence , was 21 , 700 .
	manualset3
178267	4	411064	13	NULL	NULL	0	NULL	21 , 700	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weight of methyltransferase , calculated from the predicted amino acid sequence , was 21 , 700 .
	manualset3
178268	1	411065	13	NULL	NULL	0	NULL	molecular weight	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weight was estimated to be 84000 by Sephadex G-200 molecular-sieve chromatography .
	manualset3
178269	2	411065	13	NULL	NULL	0	NULL	 84000	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weight was estimated to be 84000 by Sephadex G-200 molecular-sieve chromatography .
	manualset3
178270	3	411065	13	NULL	NULL	0	NULL	Sephadex G-200 molecular-sieve chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weight was estimated to be 84000 by Sephadex G-200 molecular-sieve chromatography .
	manualset3
178271	1	411066	13	NULL	NULL	0	NULL	molecular weights 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weights determined by gel electrophoresis in the presence of sodium dodecylsulfate and dithiothreitol ( 125 000 and 73 000 ) are in reasonable agreement with those obtained by gel filtration in 5 M guanidine-HC1 ( 125000 and 64000 ) .
	manualset3
178272	2	411066	13	NULL	NULL	0	NULL	gel electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weights determined by gel electrophoresis in the presence of sodium dodecylsulfate and dithiothreitol ( 125 000 and 73 000 ) are in reasonable agreement with those obtained by gel filtration in 5 M guanidine-HC1 ( 125000 and 64000 ) .
	manualset3
178273	3	411066	13	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weights determined by gel electrophoresis in the presence of sodium dodecylsulfate and dithiothreitol ( 125 000 and 73 000 ) are in reasonable agreement with those obtained by gel filtration in 5 M guanidine-HC1 ( 125000 and 64000 ) .
	manualset3
178274	4	411066	13	NULL	NULL	0	NULL	sodium dodecylsulfate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weights determined by gel electrophoresis in the presence of sodium dodecylsulfate and dithiothreitol ( 125 000 and 73 000 ) are in reasonable agreement with those obtained by gel filtration in 5 M guanidine-HC1 ( 125000 and 64000 ) .
	manualset3
178275	5	411066	13	NULL	NULL	0	NULL	dithiothreitol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weights determined by gel electrophoresis in the presence of sodium dodecylsulfate and dithiothreitol ( 125 000 and 73 000 ) are in reasonable agreement with those obtained by gel filtration in 5 M guanidine-HC1 ( 125000 and 64000 ) .
	manualset3
178276	6	411066	13	NULL	NULL	0	NULL	125 000	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weights determined by gel electrophoresis in the presence of sodium dodecylsulfate and dithiothreitol ( 125 000 and 73 000 ) are in reasonable agreement with those obtained by gel filtration in 5 M guanidine-HC1 ( 125000 and 64000 ) .
	manualset3
178277	7	411066	13	NULL	NULL	0	NULL	73 000	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weights determined by gel electrophoresis in the presence of sodium dodecylsulfate and dithiothreitol ( 125 000 and 73 000 ) are in reasonable agreement with those obtained by gel filtration in 5 M guanidine-HC1 ( 125000 and 64000 ) .
	manualset3
178278	8	411066	13	NULL	NULL	0	NULL	agreement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weights determined by gel electrophoresis in the presence of sodium dodecylsulfate and dithiothreitol ( 125 000 and 73 000 ) are in reasonable agreement with those obtained by gel filtration in 5 M guanidine-HC1 ( 125000 and 64000 ) .
	manualset3
178279	9	411066	13	NULL	NULL	0	NULL	gel filtration	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weights determined by gel electrophoresis in the presence of sodium dodecylsulfate and dithiothreitol ( 125 000 and 73 000 ) are in reasonable agreement with those obtained by gel filtration in 5 M guanidine-HC1 ( 125000 and 64000 ) .
	manualset3
178280	10	411066	13	NULL	NULL	0	NULL	5 M guanidine-HC1	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weights determined by gel electrophoresis in the presence of sodium dodecylsulfate and dithiothreitol ( 125 000 and 73 000 ) are in reasonable agreement with those obtained by gel filtration in 5 M guanidine-HC1 ( 125000 and 64000 ) .
	manualset3
178281	11	411066	13	NULL	NULL	0	NULL	 125000	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weights determined by gel electrophoresis in the presence of sodium dodecylsulfate and dithiothreitol ( 125 000 and 73 000 ) are in reasonable agreement with those obtained by gel filtration in 5 M guanidine-HC1 ( 125000 and 64000 ) .
	manualset3
178282	12	411066	13	NULL	NULL	0	NULL	64000	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weights determined by gel electrophoresis in the presence of sodium dodecylsulfate and dithiothreitol ( 125 000 and 73 000 ) are in reasonable agreement with those obtained by gel filtration in 5 M guanidine-HC1 ( 125000 and 64000 ) .
	manualset3
178283	1	411067	13	NULL	NULL	0	NULL	molecule 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecule contains ambroxol , which facilitates various steps in the biosynthesis of pulmonary surfactant , theophylline-7 acetic acid whose carrier function raises blood levels of ambroxol , thus rapidly and intensely stimulating surfactant production .
	manualset3
178284	2	411067	13	NULL	NULL	NULL	NULL	ambroxol	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The molecule contains ambroxol , which facilitates various steps in the biosynthesis of pulmonary surfactant , theophylline-7 acetic acid whose carrier function raises blood levels of ambroxol , thus rapidly and intensely stimulating surfactant production .
	manualset3
178285	3	411067	13	NULL	NULL	0	NULL	various steps	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecule contains ambroxol , which facilitates various steps in the biosynthesis of pulmonary surfactant , theophylline-7 acetic acid whose carrier function raises blood levels of ambroxol , thus rapidly and intensely stimulating surfactant production .
	manualset3
178286	4	411067	13	NULL	NULL	0	NULL	biosynthesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecule contains ambroxol , which facilitates various steps in the biosynthesis of pulmonary surfactant , theophylline-7 acetic acid whose carrier function raises blood levels of ambroxol , thus rapidly and intensely stimulating surfactant production .
	manualset3
178287	5	411067	13	NULL	NULL	0	NULL	pulmonary surfactant	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecule contains ambroxol , which facilitates various steps in the biosynthesis of pulmonary surfactant , theophylline-7 acetic acid whose carrier function raises blood levels of ambroxol , thus rapidly and intensely stimulating surfactant production .
	manualset3
178288	6	411067	13	NULL	NULL	0	NULL	theophylline-7 acetic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecule contains ambroxol , which facilitates various steps in the biosynthesis of pulmonary surfactant , theophylline-7 acetic acid whose carrier function raises blood levels of ambroxol , thus rapidly and intensely stimulating surfactant production .
	manualset3
178289	7	411067	13	NULL	NULL	0	NULL	carrier function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecule contains ambroxol , which facilitates various steps in the biosynthesis of pulmonary surfactant , theophylline-7 acetic acid whose carrier function raises blood levels of ambroxol , thus rapidly and intensely stimulating surfactant production .
	manualset3
178290	8	411067	13	NULL	NULL	0	NULL	blood levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecule contains ambroxol , which facilitates various steps in the biosynthesis of pulmonary surfactant , theophylline-7 acetic acid whose carrier function raises blood levels of ambroxol , thus rapidly and intensely stimulating surfactant production .
	manualset3
178291	9	411067	13	NULL	NULL	0	NULL	ambroxol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecule contains ambroxol , which facilitates various steps in the biosynthesis of pulmonary surfactant , theophylline-7 acetic acid whose carrier function raises blood levels of ambroxol , thus rapidly and intensely stimulating surfactant production .
	manualset3
178292	10	411067	13	NULL	NULL	0	NULL	surfactant	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecule contains ambroxol , which facilitates various steps in the biosynthesis of pulmonary surfactant , theophylline-7 acetic acid whose carrier function raises blood levels of ambroxol , thus rapidly and intensely stimulating surfactant production .
	manualset3
178293	11	411067	13	NULL	NULL	0	NULL	production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecule contains ambroxol , which facilitates various steps in the biosynthesis of pulmonary surfactant , theophylline-7 acetic acid whose carrier function raises blood levels of ambroxol , thus rapidly and intensely stimulating surfactant production .
	manualset3
178294	1	411068	13	NULL	NULL	0	NULL	molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecules are planar chiral and , owing to the tilt angle of the nitro groups and the position of protonation , there are altogether eight conformers possible .
	manualset3
178295	2	411068	13	NULL	NULL	0	NULL	 tilt angle 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecules are planar chiral and , owing to the tilt angle of the nitro groups and the position of protonation , there are altogether eight conformers possible .
	manualset3
178296	3	411068	13	NULL	NULL	0	NULL	nitro groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecules are planar chiral and , owing to the tilt angle of the nitro groups and the position of protonation , there are altogether eight conformers possible .
	manualset3
178297	4	411068	13	NULL	NULL	0	NULL	position	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecules are planar chiral and , owing to the tilt angle of the nitro groups and the position of protonation , there are altogether eight conformers possible .
	manualset3
178298	5	411068	13	NULL	NULL	0	NULL	protonation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecules are planar chiral and , owing to the tilt angle of the nitro groups and the position of protonation , there are altogether eight conformers possible .
	manualset3
178299	6	411068	13	NULL	NULL	0	NULL	eight conformers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecules are planar chiral and , owing to the tilt angle of the nitro groups and the position of protonation , there are altogether eight conformers possible .
	manualset3
178300	1	411069	13	NULL	NULL	0	NULL	money	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The money was collected in a nationwide campaign in an effort to express Viet Nam 's sympathy for Cubans who face difficult living conditions due to the US embargo .
	manualset3
178301	2	411069	13	NULL	NULL	0	NULL	nationwide campaign 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The money was collected in a nationwide campaign in an effort to express Viet Nam 's sympathy for Cubans who face difficult living conditions due to the US embargo .
	manualset3
178302	3	411069	13	NULL	NULL	0	NULL	effort	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The money was collected in a nationwide campaign in an effort to express Viet Nam 's sympathy for Cubans who face difficult living conditions due to the US embargo .
	manualset3
178303	4	411069	13	NULL	NULL	0	NULL	Viet Nam 's sympathy 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The money was collected in a nationwide campaign in an effort to express Viet Nam 's sympathy for Cubans who face difficult living conditions due to the US embargo .
	manualset3
178304	5	411069	13	NULL	NULL	0	NULL	Cubans	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The money was collected in a nationwide campaign in an effort to express Viet Nam 's sympathy for Cubans who face difficult living conditions due to the US embargo .
	manualset3
178305	6	411069	13	NULL	NULL	0	NULL	living conditions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The money was collected in a nationwide campaign in an effort to express Viet Nam 's sympathy for Cubans who face difficult living conditions due to the US embargo .
	manualset3
178306	7	411069	13	NULL	NULL	0	NULL	US embargo	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The money was collected in a nationwide campaign in an effort to express Viet Nam 's sympathy for Cubans who face difficult living conditions due to the US embargo .
	manualset3
178307	1	411070	13	NULL	NULL	0	NULL	monoexponential pattern 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The monoexponential pattern of restitution was seen with model-independent descriptors of relaxation as well as with tau .
	manualset3
178308	2	411070	13	NULL	NULL	0	NULL	restitution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The monoexponential pattern of restitution was seen with model-independent descriptors of relaxation as well as with tau .
	manualset3
178309	3	411070	13	NULL	NULL	0	NULL	descriptors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The monoexponential pattern of restitution was seen with model-independent descriptors of relaxation as well as with tau .
	manualset3
178310	4	411070	13	NULL	NULL	0	NULL	 relaxation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The monoexponential pattern of restitution was seen with model-independent descriptors of relaxation as well as with tau .
	manualset3
178311	5	411070	13	NULL	NULL	0	NULL	tau 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The monoexponential pattern of restitution was seen with model-independent descriptors of relaxation as well as with tau .
	manualset3
178312	1	411071	13	NULL	NULL	0	NULL	monolayer lattice structures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The monolayer lattice structures of stearic acid , 1-hexadecanol , DPPC and DPPA , obtained in this way conform to the corresponding lattice structures determined previously by other authors using GIXD .
	manualset3
178313	2	411071	13	NULL	NULL	0	NULL	stearic acid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The monolayer lattice structures of stearic acid , 1-hexadecanol , DPPC and DPPA , obtained in this way conform to the corresponding lattice structures determined previously by other authors using GIXD .
	manualset3
178314	3	411071	13	NULL	NULL	0	NULL	1-hexadecanol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The monolayer lattice structures of stearic acid , 1-hexadecanol , DPPC and DPPA , obtained in this way conform to the corresponding lattice structures determined previously by other authors using GIXD .
	manualset3
178315	4	411071	13	NULL	NULL	0	NULL	DPPC 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The monolayer lattice structures of stearic acid , 1-hexadecanol , DPPC and DPPA , obtained in this way conform to the corresponding lattice structures determined previously by other authors using GIXD .
	manualset3
178316	5	411071	13	NULL	NULL	0	NULL	DPPA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The monolayer lattice structures of stearic acid , 1-hexadecanol , DPPC and DPPA , obtained in this way conform to the corresponding lattice structures determined previously by other authors using GIXD .
	manualset3
178317	6	411071	13	NULL	NULL	0	NULL	way	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The monolayer lattice structures of stearic acid , 1-hexadecanol , DPPC and DPPA , obtained in this way conform to the corresponding lattice structures determined previously by other authors using GIXD .
	manualset3
178318	7	411071	13	NULL	NULL	0	NULL	lattice structures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The monolayer lattice structures of stearic acid , 1-hexadecanol , DPPC and DPPA , obtained in this way conform to the corresponding lattice structures determined previously by other authors using GIXD .
	manualset3
178319	8	411071	13	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The monolayer lattice structures of stearic acid , 1-hexadecanol , DPPC and DPPA , obtained in this way conform to the corresponding lattice structures determined previously by other authors using GIXD .
	manualset3
178320	9	411071	13	NULL	NULL	0	NULL	GIXD 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The monolayer lattice structures of stearic acid , 1-hexadecanol , DPPC and DPPA , obtained in this way conform to the corresponding lattice structures determined previously by other authors using GIXD .
	manualset3
178321	1	411072	13	NULL	NULL	0	NULL	variant	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A variant of this , adopts a newer set of fluorophors , also of the Cy3 and Cy5 type , reacting on Cys residues , via a strategy of `` saturation labeling '' .
	manualset3
178322	2	411072	13	NULL	NULL	0	NULL	newer set	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A variant of this , adopts a newer set of fluorophors , also of the Cy3 and Cy5 type , reacting on Cys residues , via a strategy of `` saturation labeling '' .
	manualset3
178323	3	411072	13	NULL	NULL	0	NULL	fluorophors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A variant of this , adopts a newer set of fluorophors , also of the Cy3 and Cy5 type , reacting on Cys residues , via a strategy of `` saturation labeling '' .
	manualset3
178324	4	411072	13	NULL	NULL	0	NULL	Cy3 type	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A variant of this , adopts a newer set of fluorophors , also of the Cy3 and Cy5 type , reacting on Cys residues , via a strategy of `` saturation labeling '' .
	manualset3
178325	5	411072	13	NULL	NULL	0	NULL	Cy5 type	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A variant of this , adopts a newer set of fluorophors , also of the Cy3 and Cy5 type , reacting on Cys residues , via a strategy of `` saturation labeling '' .
	manualset3
178326	6	411072	13	NULL	NULL	0	NULL	Cys residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A variant of this , adopts a newer set of fluorophors , also of the Cy3 and Cy5 type , reacting on Cys residues , via a strategy of `` saturation labeling '' .
	manualset3
178327	7	411072	13	NULL	NULL	0	NULL	strategy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A variant of this , adopts a newer set of fluorophors , also of the Cy3 and Cy5 type , reacting on Cys residues , via a strategy of `` saturation labeling '' .
	manualset3
178328	8	411072	13	NULL	NULL	0	NULL	saturation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A variant of this , adopts a newer set of fluorophors , also of the Cy3 and Cy5 type , reacting on Cys residues , via a strategy of `` saturation labeling '' .
	manualset3
178329	1	411073	13	NULL	NULL	0	NULL	morbidity rate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The morbidity rate of closed reduction is lower but , with the advent of modern anaesthesia and antibiotics , open surgery has become more frequent .
	manualset3
178330	2	411073	13	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The morbidity rate of closed reduction is lower but , with the advent of modern anaesthesia and antibiotics , open surgery has become more frequent .
	manualset3
178331	3	411073	13	NULL	NULL	0	NULL	modern anaesthesia	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The morbidity rate of closed reduction is lower but , with the advent of modern anaesthesia and antibiotics , open surgery has become more frequent .
	manualset3
178332	4	411073	13	NULL	NULL	0	NULL	antibiotics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The morbidity rate of closed reduction is lower but , with the advent of modern anaesthesia and antibiotics , open surgery has become more frequent .
	manualset3
178333	5	411073	13	NULL	NULL	0	NULL	open surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The morbidity rate of closed reduction is lower but , with the advent of modern anaesthesia and antibiotics , open surgery has become more frequent .
	manualset3
178334	1	411074	13	NULL	NULL	NULL	NULL	hydrophobic bile acids 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The more hydrophobic bile acids , chenodeoxycholic acid and deoxycholic acid , also produced a strong inhibition of 57 % and 76 % respectively , whereas the hydrophilic beta-muricholic acid was not active .
	manualset3
178335	2	411074	13	NULL	NULL	0	NULL	chenodeoxycholic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The more hydrophobic bile acids , chenodeoxycholic acid and deoxycholic acid , also produced a strong inhibition of 57 % and 76 % respectively , whereas the hydrophilic beta-muricholic acid was not active .
	manualset3
178336	3	411074	13	NULL	NULL	0	NULL	deoxycholic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The more hydrophobic bile acids , chenodeoxycholic acid and deoxycholic acid , also produced a strong inhibition of 57 % and 76 % respectively , whereas the hydrophilic beta-muricholic acid was not active .
	manualset3
178337	4	411074	13	NULL	NULL	0	NULL	inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The more hydrophobic bile acids , chenodeoxycholic acid and deoxycholic acid , also produced a strong inhibition of 57 % and 76 % respectively , whereas the hydrophilic beta-muricholic acid was not active .
	manualset3
178338	5	411074	13	NULL	NULL	0	NULL	57 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The more hydrophobic bile acids , chenodeoxycholic acid and deoxycholic acid , also produced a strong inhibition of 57 % and 76 % respectively , whereas the hydrophilic beta-muricholic acid was not active .
	manualset3
178339	6	411074	13	NULL	NULL	0	NULL	76 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The more hydrophobic bile acids , chenodeoxycholic acid and deoxycholic acid , also produced a strong inhibition of 57 % and 76 % respectively , whereas the hydrophilic beta-muricholic acid was not active .
	manualset3
178340	7	411074	13	NULL	NULL	0	NULL	hydrophilic beta-muricholic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The more hydrophobic bile acids , chenodeoxycholic acid and deoxycholic acid , also produced a strong inhibition of 57 % and 76 % respectively , whereas the hydrophilic beta-muricholic acid was not active .
	manualset3
178341	1	411075	13	NULL	NULL	0	NULL	specific signs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The more specific signs of bowel congestion and necrosis ( i.e. , a narrow rigid loop or intramural gas ) were seen in 10 % and 2 % of the cases , respectively .
	manualset3
178342	2	411075	13	NULL	NULL	0	NULL	bowel congestion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The more specific signs of bowel congestion and necrosis ( i.e. , a narrow rigid loop or intramural gas ) were seen in 10 % and 2 % of the cases , respectively .
	manualset3
178343	3	411075	13	NULL	NULL	0	NULL	necrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The more specific signs of bowel congestion and necrosis ( i.e. , a narrow rigid loop or intramural gas ) were seen in 10 % and 2 % of the cases , respectively .
	manualset3
178344	4	411075	13	NULL	NULL	0	NULL	narrow rigid loop	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The more specific signs of bowel congestion and necrosis ( i.e. , a narrow rigid loop or intramural gas ) were seen in 10 % and 2 % of the cases , respectively .
	manualset3
178345	5	411075	13	NULL	NULL	0	NULL	 intramural gas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The more specific signs of bowel congestion and necrosis ( i.e. , a narrow rigid loop or intramural gas ) were seen in 10 % and 2 % of the cases , respectively .
	manualset3
178346	6	411075	13	NULL	NULL	0	NULL	10 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The more specific signs of bowel congestion and necrosis ( i.e. , a narrow rigid loop or intramural gas ) were seen in 10 % and 2 % of the cases , respectively .
	manualset3
178347	7	411075	13	NULL	NULL	0	NULL	2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The more specific signs of bowel congestion and necrosis ( i.e. , a narrow rigid loop or intramural gas ) were seen in 10 % and 2 % of the cases , respectively .
	manualset3
178348	8	411075	13	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The more specific signs of bowel congestion and necrosis ( i.e. , a narrow rigid loop or intramural gas ) were seen in 10 % and 2 % of the cases , respectively .
	manualset3
178349	1	411076	13	NULL	NULL	0	NULL	morphologic patterns	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphologic patterns of local recurrence on CEUS were in concordance with those found on MDCT in all lesions .
	manualset3
178350	2	411076	13	NULL	NULL	0	NULL	local recurrence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphologic patterns of local recurrence on CEUS were in concordance with those found on MDCT in all lesions .
	manualset3
178351	3	411076	13	NULL	NULL	0	NULL	CEUS	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphologic patterns of local recurrence on CEUS were in concordance with those found on MDCT in all lesions .
	manualset3
178352	4	411076	13	NULL	NULL	0	NULL	concordance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphologic patterns of local recurrence on CEUS were in concordance with those found on MDCT in all lesions .
	manualset3
178353	5	411076	13	NULL	NULL	0	NULL	MDCT 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphologic patterns of local recurrence on CEUS were in concordance with those found on MDCT in all lesions .
	manualset3
178354	6	411076	13	NULL	NULL	0	NULL	 lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphologic patterns of local recurrence on CEUS were in concordance with those found on MDCT in all lesions .
	manualset3
178355	1	411077	13	NULL	NULL	0	NULL	morphological alterations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological and functional alterations along the epididymal duct and lack of spermatozoa within the lumen after deslorelin treatment indicate that a potent GnRH agonist is likely responsible for an impairment of the microenvironment created by epididymal cells for sperm maturation and their storage .
	manualset3
178356	2	411077	13	NULL	NULL	0	NULL	functional alterations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological and functional alterations along the epididymal duct and lack of spermatozoa within the lumen after deslorelin treatment indicate that a potent GnRH agonist is likely responsible for an impairment of the microenvironment created by epididymal cells for sperm maturation and their storage .
	manualset3
178357	3	411077	13	NULL	NULL	0	NULL	epididymal duct	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological and functional alterations along the epididymal duct and lack of spermatozoa within the lumen after deslorelin treatment indicate that a potent GnRH agonist is likely responsible for an impairment of the microenvironment created by epididymal cells for sperm maturation and their storage .
	manualset3
178358	4	411077	13	NULL	NULL	0	NULL	lack of spermatozoa 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological and functional alterations along the epididymal duct and lack of spermatozoa within the lumen after deslorelin treatment indicate that a potent GnRH agonist is likely responsible for an impairment of the microenvironment created by epididymal cells for sperm maturation and their storage .
	manualset3
178359	5	411077	13	NULL	NULL	0	NULL	lumen 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological and functional alterations along the epididymal duct and lack of spermatozoa within the lumen after deslorelin treatment indicate that a potent GnRH agonist is likely responsible for an impairment of the microenvironment created by epididymal cells for sperm maturation and their storage .
	manualset3
178360	6	411077	13	NULL	NULL	0	NULL	deslorelin treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological and functional alterations along the epididymal duct and lack of spermatozoa within the lumen after deslorelin treatment indicate that a potent GnRH agonist is likely responsible for an impairment of the microenvironment created by epididymal cells for sperm maturation and their storage .
	manualset3
178361	7	411077	13	NULL	NULL	0	NULL	GnRH agonist	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological and functional alterations along the epididymal duct and lack of spermatozoa within the lumen after deslorelin treatment indicate that a potent GnRH agonist is likely responsible for an impairment of the microenvironment created by epididymal cells for sperm maturation and their storage .
	manualset3
178362	8	411077	13	NULL	NULL	0	NULL	 impairment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological and functional alterations along the epididymal duct and lack of spermatozoa within the lumen after deslorelin treatment indicate that a potent GnRH agonist is likely responsible for an impairment of the microenvironment created by epididymal cells for sperm maturation and their storage .
	manualset3
178363	9	411077	13	NULL	NULL	0	NULL	microenvironment	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological and functional alterations along the epididymal duct and lack of spermatozoa within the lumen after deslorelin treatment indicate that a potent GnRH agonist is likely responsible for an impairment of the microenvironment created by epididymal cells for sperm maturation and their storage .
	manualset3
178364	10	411077	13	NULL	NULL	0	NULL	epididymal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological and functional alterations along the epididymal duct and lack of spermatozoa within the lumen after deslorelin treatment indicate that a potent GnRH agonist is likely responsible for an impairment of the microenvironment created by epididymal cells for sperm maturation and their storage .
	manualset3
178365	11	411077	13	NULL	NULL	0	NULL	sperm maturation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological and functional alterations along the epididymal duct and lack of spermatozoa within the lumen after deslorelin treatment indicate that a potent GnRH agonist is likely responsible for an impairment of the microenvironment created by epididymal cells for sperm maturation and their storage .
	manualset3
178366	12	411077	13	NULL	NULL	0	NULL	storage 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological and functional alterations along the epididymal duct and lack of spermatozoa within the lumen after deslorelin treatment indicate that a potent GnRH agonist is likely responsible for an impairment of the microenvironment created by epididymal cells for sperm maturation and their storage .
	manualset3
178367	1	411078	13	NULL	NULL	0	NULL	morphological changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological changes observed clearly show that ceftibuten has a greater affinity for and impairs the function of penicillin-binding protein 3 ( involved in synthesis of peptidoglycan for cross walls ) more than other cephalosporins , such as cephaloridine or cefoxitin .
	manualset3
178368	2	411078	13	NULL	NULL	0	NULL	 ceftibuten	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological changes observed clearly show that ceftibuten has a greater affinity for and impairs the function of penicillin-binding protein 3 ( involved in synthesis of peptidoglycan for cross walls ) more than other cephalosporins , such as cephaloridine or cefoxitin .
	manualset3
178369	3	411078	13	NULL	NULL	0	NULL	affinity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological changes observed clearly show that ceftibuten has a greater affinity for and impairs the function of penicillin-binding protein 3 ( involved in synthesis of peptidoglycan for cross walls ) more than other cephalosporins , such as cephaloridine or cefoxitin .
	manualset3
178370	4	411078	13	NULL	NULL	0	NULL	function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological changes observed clearly show that ceftibuten has a greater affinity for and impairs the function of penicillin-binding protein 3 ( involved in synthesis of peptidoglycan for cross walls ) more than other cephalosporins , such as cephaloridine or cefoxitin .
	manualset3
178371	5	411078	13	NULL	NULL	0	NULL	penicillin-binding protein 3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological changes observed clearly show that ceftibuten has a greater affinity for and impairs the function of penicillin-binding protein 3 ( involved in synthesis of peptidoglycan for cross walls ) more than other cephalosporins , such as cephaloridine or cefoxitin .
	manualset3
178372	6	411078	13	NULL	NULL	0	NULL	synthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological changes observed clearly show that ceftibuten has a greater affinity for and impairs the function of penicillin-binding protein 3 ( involved in synthesis of peptidoglycan for cross walls ) more than other cephalosporins , such as cephaloridine or cefoxitin .
	manualset3
178373	7	411078	13	NULL	NULL	0	NULL	peptidoglycan	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological changes observed clearly show that ceftibuten has a greater affinity for and impairs the function of penicillin-binding protein 3 ( involved in synthesis of peptidoglycan for cross walls ) more than other cephalosporins , such as cephaloridine or cefoxitin .
	manualset3
178374	8	411078	13	NULL	NULL	0	NULL	 cross walls	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological changes observed clearly show that ceftibuten has a greater affinity for and impairs the function of penicillin-binding protein 3 ( involved in synthesis of peptidoglycan for cross walls ) more than other cephalosporins , such as cephaloridine or cefoxitin .
	manualset3
178375	9	411078	13	NULL	NULL	0	NULL	cephalosporins	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological changes observed clearly show that ceftibuten has a greater affinity for and impairs the function of penicillin-binding protein 3 ( involved in synthesis of peptidoglycan for cross walls ) more than other cephalosporins , such as cephaloridine or cefoxitin .
	manualset3
178376	10	411078	13	NULL	NULL	0	NULL	cephaloridine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological changes observed clearly show that ceftibuten has a greater affinity for and impairs the function of penicillin-binding protein 3 ( involved in synthesis of peptidoglycan for cross walls ) more than other cephalosporins , such as cephaloridine or cefoxitin .
	manualset3
178377	11	411078	13	NULL	NULL	0	NULL	cefoxitin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological changes observed clearly show that ceftibuten has a greater affinity for and impairs the function of penicillin-binding protein 3 ( involved in synthesis of peptidoglycan for cross walls ) more than other cephalosporins , such as cephaloridine or cefoxitin .
	manualset3
178378	1	411079	13	NULL	NULL	NULL	NULL	variety	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A variety of cell types including hepatic stellate cells , alternatively activated macrophages and regulatory T-cells have also been implicated in the pathogenesis of schistosomiasis .
	manualset3
178379	2	411079	13	NULL	NULL	0	NULL	cell types	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A variety of cell types including hepatic stellate cells , alternatively activated macrophages and regulatory T-cells have also been implicated in the pathogenesis of schistosomiasis .
	manualset3
178380	3	411079	13	NULL	NULL	0	NULL	hepatic stellate cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A variety of cell types including hepatic stellate cells , alternatively activated macrophages and regulatory T-cells have also been implicated in the pathogenesis of schistosomiasis .
	manualset3
178381	4	411079	13	NULL	NULL	0	NULL	macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A variety of cell types including hepatic stellate cells , alternatively activated macrophages and regulatory T-cells have also been implicated in the pathogenesis of schistosomiasis .
	manualset3
178382	5	411079	13	NULL	NULL	0	NULL	regulatory T-cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A variety of cell types including hepatic stellate cells , alternatively activated macrophages and regulatory T-cells have also been implicated in the pathogenesis of schistosomiasis .
	manualset3
178383	6	411079	13	NULL	NULL	0	NULL	pathogenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A variety of cell types including hepatic stellate cells , alternatively activated macrophages and regulatory T-cells have also been implicated in the pathogenesis of schistosomiasis .
	manualset3
178384	7	411079	13	NULL	NULL	0	NULL	schistosomiasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A variety of cell types including hepatic stellate cells , alternatively activated macrophages and regulatory T-cells have also been implicated in the pathogenesis of schistosomiasis .
	manualset3
178385	1	411080	13	NULL	NULL	0	NULL	morphology of cysts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphology of cysts , as it appears in ultrasound images , is currently used for classification of ovarian pathologies .
	manualset3
178386	2	411080	13	NULL	NULL	0	NULL	ultrasound images	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphology of cysts , as it appears in ultrasound images , is currently used for classification of ovarian pathologies .
	manualset3
178387	3	411080	13	NULL	NULL	0	NULL	 classification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphology of cysts , as it appears in ultrasound images , is currently used for classification of ovarian pathologies .
	manualset3
178388	4	411080	13	NULL	NULL	0	NULL	ovarian pathologies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphology of cysts , as it appears in ultrasound images , is currently used for classification of ovarian pathologies .
	manualset3
178389	1	411081	13	NULL	NULL	0	NULL	morphology	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphology of the microspheres was evaluated using a scanning electron microscope , which showed a spherical shape with smooth surface .
	manualset3
178390	2	411081	13	NULL	NULL	0	NULL	microspheres	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphology of the microspheres was evaluated using a scanning electron microscope , which showed a spherical shape with smooth surface .
	manualset3
178391	3	411081	13	NULL	NULL	0	NULL	scanning electron microscope	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphology of the microspheres was evaluated using a scanning electron microscope , which showed a spherical shape with smooth surface .
	manualset3
178392	4	411081	13	NULL	NULL	0	NULL	spherical shape 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphology of the microspheres was evaluated using a scanning electron microscope , which showed a spherical shape with smooth surface .
	manualset3
178393	5	411081	13	NULL	NULL	0	NULL	smooth surface	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphology of the microspheres was evaluated using a scanning electron microscope , which showed a spherical shape with smooth surface .
	manualset3
178394	1	411082	13	NULL	NULL	0	NULL	 mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The mortality was 35 % in vehicle-treated , 40 % in PAG-treated , and 27.5 % in NaHS-treated ( P & lt ; 0.05 vs. vehicle ) groups .
	manualset3
178395	2	411082	13	NULL	NULL	0	NULL	35 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mortality was 35 % in vehicle-treated , 40 % in PAG-treated , and 27.5 % in NaHS-treated ( P & lt ; 0.05 vs. vehicle ) groups .
	manualset3
178396	3	411082	13	NULL	NULL	0	NULL	40 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mortality was 35 % in vehicle-treated , 40 % in PAG-treated , and 27.5 % in NaHS-treated ( P & lt ; 0.05 vs. vehicle ) groups .
	manualset3
178397	4	411082	13	NULL	NULL	0	NULL	PAG-treated groups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The mortality was 35 % in vehicle-treated , 40 % in PAG-treated , and 27.5 % in NaHS-treated ( P & lt ; 0.05 vs. vehicle ) groups .
	manualset3
178398	5	411082	13	NULL	NULL	0	NULL	27.5 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mortality was 35 % in vehicle-treated , 40 % in PAG-treated , and 27.5 % in NaHS-treated ( P & lt ; 0.05 vs. vehicle ) groups .
	manualset3
178399	6	411082	13	NULL	NULL	0	NULL	NaHS-treated groups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The mortality was 35 % in vehicle-treated , 40 % in PAG-treated , and 27.5 % in NaHS-treated ( P & lt ; 0.05 vs. vehicle ) groups .
	manualset3
178400	7	411082	13	NULL	NULL	0	NULL	P & lt ; 0.05 vs. vehicle	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mortality was 35 % in vehicle-treated , 40 % in PAG-treated , and 27.5 % in NaHS-treated ( P & lt ; 0.05 vs. vehicle ) groups .
	manualset3
178401	1	411083	13	NULL	NULL	0	NULL	extract	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The most active extract obtained from mammary gland tissue was chromatographed and the TGF activity shown to be coeluting with EGF receptor-competing activity .
	manualset3
178402	2	411083	13	NULL	NULL	0	NULL	mammary gland tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The most active extract obtained from mammary gland tissue was chromatographed and the TGF activity shown to be coeluting with EGF receptor-competing activity .
	manualset3
178403	3	411083	13	NULL	NULL	0	NULL	TGF activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The most active extract obtained from mammary gland tissue was chromatographed and the TGF activity shown to be coeluting with EGF receptor-competing activity .
	manualset3
178404	4	411083	13	NULL	NULL	0	NULL	EGF receptor-competing activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The most active extract obtained from mammary gland tissue was chromatographed and the TGF activity shown to be coeluting with EGF receptor-competing activity .
	manualset3
178405	1	411084	13	NULL	NULL	0	NULL	characteristic feature	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The most characteristic feature of osteoclasts is multinucleation resulting from cell-cell fusion of mononuclear osteoclasts .
	manualset3
178406	2	411084	13	NULL	NULL	0	NULL	osteoclasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The most characteristic feature of osteoclasts is multinucleation resulting from cell-cell fusion of mononuclear osteoclasts .
	manualset3
178407	3	411084	13	NULL	NULL	0	NULL	 cell-cell fusion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The most characteristic feature of osteoclasts is multinucleation resulting from cell-cell fusion of mononuclear osteoclasts .
	manualset3
178408	4	411084	13	NULL	NULL	0	NULL	mononuclear osteoclasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The most characteristic feature of osteoclasts is multinucleation resulting from cell-cell fusion of mononuclear osteoclasts .
	manualset3
178409	5	411084	13	NULL	NULL	0	NULL	 multinucleation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The most characteristic feature of osteoclasts is multinucleation resulting from cell-cell fusion of mononuclear osteoclasts .
	manualset3
178410	1	411085	13	NULL	NULL	0	NULL	cause of death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common cause of death ( 60 % ) was meningitis .
	manualset3
178411	2	411085	13	NULL	NULL	0	NULL	60 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common cause of death ( 60 % ) was meningitis .
	manualset3
178412	3	411085	13	NULL	NULL	0	NULL	meningitis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common cause of death ( 60 % ) was meningitis .
	manualset3
178413	1	411086	13	NULL	NULL	0	NULL	common cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common cause of fetal seizures was congenital anomalies ( seven of 13 ) , mainly of the central nervous system ( six of seven ) .
	manualset3
178414	2	411086	13	NULL	NULL	0	NULL	fetal seizures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common cause of fetal seizures was congenital anomalies ( seven of 13 ) , mainly of the central nervous system ( six of seven ) .
	manualset3
178415	3	411086	13	NULL	NULL	0	NULL	congenital anomalies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common cause of fetal seizures was congenital anomalies ( seven of 13 ) , mainly of the central nervous system ( six of seven ) .
	manualset3
178416	4	411086	13	NULL	NULL	0	NULL	seven of 13	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common cause of fetal seizures was congenital anomalies ( seven of 13 ) , mainly of the central nervous system ( six of seven ) .
	manualset3
178417	5	411086	13	NULL	NULL	0	NULL	 central nervous system 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common cause of fetal seizures was congenital anomalies ( seven of 13 ) , mainly of the central nervous system ( six of seven ) .
	manualset3
178418	6	411086	13	NULL	NULL	0	NULL	six of seven	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common cause of fetal seizures was congenital anomalies ( seven of 13 ) , mainly of the central nervous system ( six of seven ) .
	manualset3
178419	1	411087	13	NULL	NULL	0	NULL	variety	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A variety of new agents and combinations have been investigated in the treatment of NSCLC .
	manualset3
178420	2	411087	13	NULL	NULL	0	NULL	new agents 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A variety of new agents and combinations have been investigated in the treatment of NSCLC .
	manualset3
178421	3	411087	13	NULL	NULL	0	NULL	combinations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A variety of new agents and combinations have been investigated in the treatment of NSCLC .
	manualset3
178422	4	411087	13	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A variety of new agents and combinations have been investigated in the treatment of NSCLC .
	manualset3
178423	5	411087	13	NULL	NULL	0	NULL	NSCLC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A variety of new agents and combinations have been investigated in the treatment of NSCLC .
	manualset3
178424	1	411088	13	NULL	NULL	0	NULL	child protection concerns	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common child protection concerns were neglect , emotional maltreatment and exposure to domestic violence .
	manualset3
178425	2	411088	13	NULL	NULL	0	NULL	emotional maltreatment 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common child protection concerns were neglect , emotional maltreatment and exposure to domestic violence .
	manualset3
178426	3	411088	13	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common child protection concerns were neglect , emotional maltreatment and exposure to domestic violence .
	manualset3
178427	4	411088	13	NULL	NULL	0	NULL	domestic violence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common child protection concerns were neglect , emotional maltreatment and exposure to domestic violence .
	manualset3
178428	1	411089	13	NULL	NULL	0	NULL	complication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common complication is cardiac tamponade , which requires drainage .
	manualset3
178429	2	411089	13	NULL	NULL	0	NULL	cardiac tamponade	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common complication is cardiac tamponade , which requires drainage .
	manualset3
178430	3	411089	13	NULL	NULL	0	NULL	drainage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common complication is cardiac tamponade , which requires drainage .
	manualset3
178431	1	411090	13	NULL	NULL	0	NULL	etiologic cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common etiologic cause of thyrotoxicosis in children and adults is autoimmune Graves ' ( Basedow 's ) disease .
	manualset3
178432	2	411090	13	NULL	NULL	0	NULL	thyrotoxicosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common etiologic cause of thyrotoxicosis in children and adults is autoimmune Graves ' ( Basedow 's ) disease .
	manualset3
178433	3	411090	13	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common etiologic cause of thyrotoxicosis in children and adults is autoimmune Graves ' ( Basedow 's ) disease .
	manualset3
178434	4	411090	13	NULL	NULL	0	NULL	adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common etiologic cause of thyrotoxicosis in children and adults is autoimmune Graves ' ( Basedow 's ) disease .
	manualset3
178435	5	411090	13	NULL	NULL	0	NULL	autoimmune Graves ' ( Basedow 's ) disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common etiologic cause of thyrotoxicosis in children and adults is autoimmune Graves ' ( Basedow 's ) disease .
	manualset3
178436	1	411091	13	NULL	NULL	0	NULL	treatments	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common first-line treatments for mild to moderate disease were highpotency topical steroids ( 68 % ) followed by topical vitamin D analogs ( 41 % ) .
	manualset3
178437	2	411091	13	NULL	NULL	0	NULL	mild disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common first-line treatments for mild to moderate disease were highpotency topical steroids ( 68 % ) followed by topical vitamin D analogs ( 41 % ) .
	manualset3
178438	3	411091	13	NULL	NULL	0	NULL	moderate disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common first-line treatments for mild to moderate disease were highpotency topical steroids ( 68 % ) followed by topical vitamin D analogs ( 41 % ) .
	manualset3
178439	4	411091	13	NULL	NULL	0	NULL	topical steroids 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common first-line treatments for mild to moderate disease were highpotency topical steroids ( 68 % ) followed by topical vitamin D analogs ( 41 % ) .
	manualset3
178440	5	411091	13	NULL	NULL	0	NULL	68 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common first-line treatments for mild to moderate disease were highpotency topical steroids ( 68 % ) followed by topical vitamin D analogs ( 41 % ) .
	manualset3
178441	6	411091	13	NULL	NULL	0	NULL	topical vitamin D analogs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common first-line treatments for mild to moderate disease were highpotency topical steroids ( 68 % ) followed by topical vitamin D analogs ( 41 % ) .
	manualset3
178442	7	411091	13	NULL	NULL	0	NULL	41 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common first-line treatments for mild to moderate disease were highpotency topical steroids ( 68 % ) followed by topical vitamin D analogs ( 41 % ) .
	manualset3
178443	1	411092	13	NULL	NULL	0	NULL	events	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common initiating events are marital conflict , social isolation , loneliness , physical illness and conflicts with relatives , especially children .
	manualset3
178444	2	411092	13	NULL	NULL	0	NULL	marital conflict	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common initiating events are marital conflict , social isolation , loneliness , physical illness and conflicts with relatives , especially children .
	manualset3
178445	3	411092	13	NULL	NULL	0	NULL	social isolation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common initiating events are marital conflict , social isolation , loneliness , physical illness and conflicts with relatives , especially children .
	manualset3
178446	4	411092	13	NULL	NULL	0	NULL	loneliness 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common initiating events are marital conflict , social isolation , loneliness , physical illness and conflicts with relatives , especially children .
	manualset3
178447	5	411092	13	NULL	NULL	0	NULL	physical illness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common initiating events are marital conflict , social isolation , loneliness , physical illness and conflicts with relatives , especially children .
	manualset3
178448	6	411092	13	NULL	NULL	0	NULL	conflicts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common initiating events are marital conflict , social isolation , loneliness , physical illness and conflicts with relatives , especially children .
	manualset3
178449	7	411092	13	NULL	NULL	0	NULL	relatives	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common initiating events are marital conflict , social isolation , loneliness , physical illness and conflicts with relatives , especially children .
	manualset3
178450	8	411092	13	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common initiating events are marital conflict , social isolation , loneliness , physical illness and conflicts with relatives , especially children .
	manualset3
178451	1	411093	13	NULL	NULL	0	NULL	sexual dysfunctions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common of the sexual dysfunctions in men are premature ejaculation and impotence .
	manualset3
178452	2	411093	13	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common of the sexual dysfunctions in men are premature ejaculation and impotence .
	manualset3
178453	3	411093	13	NULL	NULL	0	NULL	premature ejaculation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common of the sexual dysfunctions in men are premature ejaculation and impotence .
	manualset3
178454	4	411093	13	NULL	NULL	0	NULL	impotence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common of the sexual dysfunctions in men are premature ejaculation and impotence .
	manualset3
178504	1	411094	13	NULL	NULL	0	NULL	reason 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common reason for poor adherence was `` frequency of administration '' , and 83.2 % of the patients preferred a once-daily administration .
	manualset3
178505	2	411094	13	NULL	NULL	0	NULL	adherence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common reason for poor adherence was `` frequency of administration '' , and 83.2 % of the patients preferred a once-daily administration .
	manualset3
178506	3	411094	13	NULL	NULL	0	NULL	frequency of administration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common reason for poor adherence was `` frequency of administration '' , and 83.2 % of the patients preferred a once-daily administration .
	manualset3
178507	4	411094	13	NULL	NULL	0	NULL	83.2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common reason for poor adherence was `` frequency of administration '' , and 83.2 % of the patients preferred a once-daily administration .
	manualset3
178508	5	411094	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common reason for poor adherence was `` frequency of administration '' , and 83.2 % of the patients preferred a once-daily administration .
	manualset3
178509	6	411094	13	NULL	NULL	0	NULL	administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common reason for poor adherence was `` frequency of administration '' , and 83.2 % of the patients preferred a once-daily administration .
	manualset3
178510	1	411095	13	NULL	NULL	0	NULL	use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common use for diagnostic thoracoscopy in pleural disease is to clarify whether or not an effusion is malignant .
	manualset3
178511	2	411095	13	NULL	NULL	0	NULL	diagnostic thoracoscopy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common use for diagnostic thoracoscopy in pleural disease is to clarify whether or not an effusion is malignant .
	manualset3
178512	3	411095	13	NULL	NULL	0	NULL	pleural disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common use for diagnostic thoracoscopy in pleural disease is to clarify whether or not an effusion is malignant .
	manualset3
178513	4	411095	13	NULL	NULL	0	NULL	effusion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common use for diagnostic thoracoscopy in pleural disease is to clarify whether or not an effusion is malignant .
	manualset3
178514	1	411096	13	NULL	NULL	0	NULL	 promise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A verbal promise should be obtained from suicidal patients that they will not commit a suicidal act for a specific period of time , e.g. until the next consultation with the doctor or until a critical point in the near future has been overcome .
	manualset3
178515	2	411096	13	NULL	NULL	0	NULL	suicidal patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A verbal promise should be obtained from suicidal patients that they will not commit a suicidal act for a specific period of time , e.g. until the next consultation with the doctor or until a critical point in the near future has been overcome .
	manualset3
178516	3	411096	13	NULL	NULL	0	NULL	suicidal act	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A verbal promise should be obtained from suicidal patients that they will not commit a suicidal act for a specific period of time , e.g. until the next consultation with the doctor or until a critical point in the near future has been overcome .
	manualset3
178517	4	411096	13	NULL	NULL	0	NULL	period of time	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A verbal promise should be obtained from suicidal patients that they will not commit a suicidal act for a specific period of time , e.g. until the next consultation with the doctor or until a critical point in the near future has been overcome .
	manualset3
178518	5	411096	13	NULL	NULL	0	NULL	consultation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A verbal promise should be obtained from suicidal patients that they will not commit a suicidal act for a specific period of time , e.g. until the next consultation with the doctor or until a critical point in the near future has been overcome .
	manualset3
178519	6	411096	13	NULL	NULL	0	NULL	doctor 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A verbal promise should be obtained from suicidal patients that they will not commit a suicidal act for a specific period of time , e.g. until the next consultation with the doctor or until a critical point in the near future has been overcome .
	manualset3
178520	7	411096	13	NULL	NULL	0	NULL	critical point 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A verbal promise should be obtained from suicidal patients that they will not commit a suicidal act for a specific period of time , e.g. until the next consultation with the doctor or until a critical point in the near future has been overcome .
	manualset3
178521	8	411096	13	NULL	NULL	0	NULL	future	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A verbal promise should be obtained from suicidal patients that they will not commit a suicidal act for a specific period of time , e.g. until the next consultation with the doctor or until a critical point in the near future has been overcome .
	manualset3
178522	1	411097	13	NULL	NULL	0	NULL	pharmacological agents 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The most commonly used pharmacological agents are - blockers and verapamil , a calcium antagonist , which are the mainstay of therapy .
	manualset3
178523	2	411097	13	NULL	NULL	0	NULL	blockers	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The most commonly used pharmacological agents are - blockers and verapamil , a calcium antagonist , which are the mainstay of therapy .
	manualset3
178524	3	411097	13	NULL	NULL	0	NULL	verapamil	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The most commonly used pharmacological agents are - blockers and verapamil , a calcium antagonist , which are the mainstay of therapy .
	manualset3
178525	4	411097	13	NULL	NULL	0	NULL	calcium antagonist	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The most commonly used pharmacological agents are - blockers and verapamil , a calcium antagonist , which are the mainstay of therapy .
	manualset3
178526	5	411097	13	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The most commonly used pharmacological agents are - blockers and verapamil , a calcium antagonist , which are the mainstay of therapy .
	manualset3
178527	1	411098	13	NULL	NULL	0	NULL	Axis-II disorder	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most diagnosed Axis-II disorder was found as to be antisocial personality disorder ( 48.6 % ) .
	manualset3
178528	2	411098	13	NULL	NULL	0	NULL	antisocial personality disorder	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most diagnosed Axis-II disorder was found as to be antisocial personality disorder ( 48.6 % ) .
	manualset3
178529	3	411098	13	NULL	NULL	0	NULL	48.6 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The most diagnosed Axis-II disorder was found as to be antisocial personality disorder ( 48.6 % ) .
	manualset3
178549	1	411099	13	NULL	NULL	0	NULL	dominant novel molecular signature	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The most dominant novel molecular signature , however , could not be identified by cultivation efforts or correlation with microscopy and , upon phylogenetic analyses , its 16S rRNA genes showed no particular close association to known cyanobacterial groups .
	manualset3
178550	2	411099	13	NULL	NULL	0	NULL	cultivation efforts 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most dominant novel molecular signature , however , could not be identified by cultivation efforts or correlation with microscopy and , upon phylogenetic analyses , its 16S rRNA genes showed no particular close association to known cyanobacterial groups .
	manualset3
178551	3	411099	13	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The most dominant novel molecular signature , however , could not be identified by cultivation efforts or correlation with microscopy and , upon phylogenetic analyses , its 16S rRNA genes showed no particular close association to known cyanobacterial groups .
	manualset3
178552	4	411099	13	NULL	NULL	0	NULL	microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The most dominant novel molecular signature , however , could not be identified by cultivation efforts or correlation with microscopy and , upon phylogenetic analyses , its 16S rRNA genes showed no particular close association to known cyanobacterial groups .
	manualset3
178553	5	411099	13	NULL	NULL	0	NULL	phylogenetic analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The most dominant novel molecular signature , however , could not be identified by cultivation efforts or correlation with microscopy and , upon phylogenetic analyses , its 16S rRNA genes showed no particular close association to known cyanobacterial groups .
	manualset3
178554	6	411099	13	NULL	NULL	0	NULL	16S rRNA genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The most dominant novel molecular signature , however , could not be identified by cultivation efforts or correlation with microscopy and , upon phylogenetic analyses , its 16S rRNA genes showed no particular close association to known cyanobacterial groups .
	manualset3
178555	7	411099	13	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The most dominant novel molecular signature , however , could not be identified by cultivation efforts or correlation with microscopy and , upon phylogenetic analyses , its 16S rRNA genes showed no particular close association to known cyanobacterial groups .
	manualset3
178556	8	411099	13	NULL	NULL	0	NULL	cyanobacterial groups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The most dominant novel molecular signature , however , could not be identified by cultivation efforts or correlation with microscopy and , upon phylogenetic analyses , its 16S rRNA genes showed no particular close association to known cyanobacterial groups .
	manualset3
178557	1	411100	13	NULL	NULL	0	NULL	regimen	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The most effective regimen in patients 61 to 70 years consisted of a combination of daunorubicin and cytosine arabinoside .
	manualset3
178558	2	411100	13	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The most effective regimen in patients 61 to 70 years consisted of a combination of daunorubicin and cytosine arabinoside .
	manualset3
178559	3	411100	13	NULL	NULL	0	NULL	 61 to 70 years	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The most effective regimen in patients 61 to 70 years consisted of a combination of daunorubicin and cytosine arabinoside .
	manualset3
178560	4	411100	13	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most effective regimen in patients 61 to 70 years consisted of a combination of daunorubicin and cytosine arabinoside .
	manualset3
178561	5	411100	13	NULL	NULL	0	NULL	daunorubicin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The most effective regimen in patients 61 to 70 years consisted of a combination of daunorubicin and cytosine arabinoside .
	manualset3
178562	6	411100	13	NULL	NULL	0	NULL	cytosine arabinoside	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The most effective regimen in patients 61 to 70 years consisted of a combination of daunorubicin and cytosine arabinoside .
	manualset3
178563	1	411101	13	NULL	NULL	0	NULL	 resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most effective resistance was induced by the two modes of administration which produced an infection involving the entire respiratory tract , i.e. , small-particle aerosol or i.n. instillation of a 200-microliter inoculum .
	manualset3
178564	2	411101	13	NULL	NULL	0	NULL	two modes	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The most effective resistance was induced by the two modes of administration which produced an infection involving the entire respiratory tract , i.e. , small-particle aerosol or i.n. instillation of a 200-microliter inoculum .
	manualset3
178565	3	411101	13	NULL	NULL	0	NULL	administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The most effective resistance was induced by the two modes of administration which produced an infection involving the entire respiratory tract , i.e. , small-particle aerosol or i.n. instillation of a 200-microliter inoculum .
	manualset3
178566	4	411101	13	NULL	NULL	0	NULL	infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most effective resistance was induced by the two modes of administration which produced an infection involving the entire respiratory tract , i.e. , small-particle aerosol or i.n. instillation of a 200-microliter inoculum .
	manualset3
178567	5	411101	13	NULL	NULL	0	NULL	 respiratory tract 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The most effective resistance was induced by the two modes of administration which produced an infection involving the entire respiratory tract , i.e. , small-particle aerosol or i.n. instillation of a 200-microliter inoculum .
	manualset3
178568	6	411101	13	NULL	NULL	0	NULL	small-particle aerosol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The most effective resistance was induced by the two modes of administration which produced an infection involving the entire respiratory tract , i.e. , small-particle aerosol or i.n. instillation of a 200-microliter inoculum .
	manualset3
178569	7	411101	13	NULL	NULL	0	NULL	instillation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most effective resistance was induced by the two modes of administration which produced an infection involving the entire respiratory tract , i.e. , small-particle aerosol or i.n. instillation of a 200-microliter inoculum .
	manualset3
178570	8	411101	13	NULL	NULL	0	NULL	200-microliter inoculum	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The most effective resistance was induced by the two modes of administration which produced an infection involving the entire respiratory tract , i.e. , small-particle aerosol or i.n. instillation of a 200-microliter inoculum .
	manualset3
178571	1	411102	13	NULL	NULL	0	NULL	topoisomerase II inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The most effective topoisomerase II inhibitor in the bis ( 2 , 6-dioxopiperazine ) series is ICRF-193 ( meso or S * , R * isomer ) , with a meso 2 , 3-butanediyl linker connecting the dioxopiperazine rings .
	manualset3
178572	2	411102	13	NULL	NULL	0	NULL	bis ( 2 , 6-dioxopiperazine ) series	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The most effective topoisomerase II inhibitor in the bis ( 2 , 6-dioxopiperazine ) series is ICRF-193 ( meso or S * , R * isomer ) , with a meso 2 , 3-butanediyl linker connecting the dioxopiperazine rings .
	manualset3
178573	3	411102	13	NULL	NULL	0	NULL	ICRF-193	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The most effective topoisomerase II inhibitor in the bis ( 2 , 6-dioxopiperazine ) series is ICRF-193 ( meso or S * , R * isomer ) , with a meso 2 , 3-butanediyl linker connecting the dioxopiperazine rings .
	manualset3
178574	4	411102	13	NULL	NULL	0	NULL	meso or S * , R * isomer 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The most effective topoisomerase II inhibitor in the bis ( 2 , 6-dioxopiperazine ) series is ICRF-193 ( meso or S * , R * isomer ) , with a meso 2 , 3-butanediyl linker connecting the dioxopiperazine rings .
	manualset3
178575	5	411102	13	NULL	NULL	0	NULL	meso 2 , 3-butanediyl linker 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The most effective topoisomerase II inhibitor in the bis ( 2 , 6-dioxopiperazine ) series is ICRF-193 ( meso or S * , R * isomer ) , with a meso 2 , 3-butanediyl linker connecting the dioxopiperazine rings .
	manualset3
178576	6	411102	13	NULL	NULL	0	NULL	dioxopiperazine rings	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The most effective topoisomerase II inhibitor in the bis ( 2 , 6-dioxopiperazine ) series is ICRF-193 ( meso or S * , R * isomer ) , with a meso 2 , 3-butanediyl linker connecting the dioxopiperazine rings .
	manualset3
178578	2	411103	13	NULL	NULL	0	NULL	gD-null virions 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The most effective were the gD-null virions , positive for gH/gL and gB .
	manualset3
178579	3	411103	13	NULL	NULL	0	NULL	gH/gL	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The most effective were the gD-null virions , positive for gH/gL and gB .
	manualset3
178580	4	411103	13	NULL	NULL	0	NULL	gB	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The most effective were the gD-null virions , positive for gH/gL and gB .
	manualset3
178581	1	411104	13	NULL	NULL	0	NULL	versatile tool 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A versatile tool for monoclonal antibody characterization .
	manualset3
178582	2	411104	13	NULL	NULL	0	NULL	monoclonal antibody 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A versatile tool for monoclonal antibody characterization .
	manualset3
178583	3	411104	13	NULL	NULL	0	NULL	characterization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A versatile tool for monoclonal antibody characterization .
	manualset3
178584	1	411105	13	NULL	NULL	0	NULL	side-effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most frequently reported side-effect was erythema , but oedema , blistering , crusting and pigment changes were also reported .
	manualset3
178585	2	411105	13	NULL	NULL	0	NULL	erythema	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most frequently reported side-effect was erythema , but oedema , blistering , crusting and pigment changes were also reported .
	manualset3
178586	3	411105	13	NULL	NULL	0	NULL	oedema	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most frequently reported side-effect was erythema , but oedema , blistering , crusting and pigment changes were also reported .
	manualset3
178587	4	411105	13	NULL	NULL	0	NULL	pigment changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most frequently reported side-effect was erythema , but oedema , blistering , crusting and pigment changes were also reported .
	manualset3
178588	1	411106	13	NULL	NULL	0	NULL	method	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The most frequently used method of diagnosing voice diseases is videostroboscopy .
	manualset3
178589	2	411106	13	NULL	NULL	0	NULL	voice diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The most frequently used method of diagnosing voice diseases is videostroboscopy .
	manualset3
178590	3	411106	13	NULL	NULL	0	NULL	videostroboscopy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The most frequently used method of diagnosing voice diseases is videostroboscopy .
	manualset3
178591	1	411107	13	NULL	NULL	0	NULL	procedures 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The most frequently used procedures -- the buried dermal flap , the Charles procedure , and the subcutaneous excision beneath flaps -- offer patients symptomatic improvement , primarily through the excision of lymphedematous subcutaneous tissue .
	manualset3
178592	2	411107	13	NULL	NULL	0	NULL	dermal flap	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The most frequently used procedures -- the buried dermal flap , the Charles procedure , and the subcutaneous excision beneath flaps -- offer patients symptomatic improvement , primarily through the excision of lymphedematous subcutaneous tissue .
	manualset3
178593	3	411107	13	NULL	NULL	0	NULL	Charles procedure 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The most frequently used procedures -- the buried dermal flap , the Charles procedure , and the subcutaneous excision beneath flaps -- offer patients symptomatic improvement , primarily through the excision of lymphedematous subcutaneous tissue .
	manualset3
178594	4	411107	13	NULL	NULL	0	NULL	subcutaneous excision 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The most frequently used procedures -- the buried dermal flap , the Charles procedure , and the subcutaneous excision beneath flaps -- offer patients symptomatic improvement , primarily through the excision of lymphedematous subcutaneous tissue .
	manualset3
178595	5	411107	13	NULL	NULL	0	NULL	flaps	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The most frequently used procedures -- the buried dermal flap , the Charles procedure , and the subcutaneous excision beneath flaps -- offer patients symptomatic improvement , primarily through the excision of lymphedematous subcutaneous tissue .
	manualset3
178596	6	411107	13	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The most frequently used procedures -- the buried dermal flap , the Charles procedure , and the subcutaneous excision beneath flaps -- offer patients symptomatic improvement , primarily through the excision of lymphedematous subcutaneous tissue .
	manualset3
178597	7	411107	13	NULL	NULL	0	NULL	symptomatic improvement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most frequently used procedures -- the buried dermal flap , the Charles procedure , and the subcutaneous excision beneath flaps -- offer patients symptomatic improvement , primarily through the excision of lymphedematous subcutaneous tissue .
	manualset3
178598	8	411107	13	NULL	NULL	0	NULL	excision	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The most frequently used procedures -- the buried dermal flap , the Charles procedure , and the subcutaneous excision beneath flaps -- offer patients symptomatic improvement , primarily through the excision of lymphedematous subcutaneous tissue .
	manualset3
178599	9	411107	13	NULL	NULL	0	NULL	lymphedematous subcutaneous tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The most frequently used procedures -- the buried dermal flap , the Charles procedure , and the subcutaneous excision beneath flaps -- offer patients symptomatic improvement , primarily through the excision of lymphedematous subcutaneous tissue .
	manualset3
178600	1	411108	13	NULL	NULL	0	NULL	group of antifungals 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important group of antifungals is the azoles ( e.g. miconazole ) , which act by inhibiting lanosterol demethylase in the sterol biosynthesis pathway .
	manualset3
178601	2	411108	13	NULL	NULL	0	NULL	azoles	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important group of antifungals is the azoles ( e.g. miconazole ) , which act by inhibiting lanosterol demethylase in the sterol biosynthesis pathway .
	manualset3
178602	3	411108	13	NULL	NULL	0	NULL	miconazole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important group of antifungals is the azoles ( e.g. miconazole ) , which act by inhibiting lanosterol demethylase in the sterol biosynthesis pathway .
	manualset3
178603	4	411108	13	NULL	NULL	0	NULL	lanosterol demethylase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important group of antifungals is the azoles ( e.g. miconazole ) , which act by inhibiting lanosterol demethylase in the sterol biosynthesis pathway .
	manualset3
178604	5	411108	13	NULL	NULL	0	NULL	sterol biosynthesis pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important group of antifungals is the azoles ( e.g. miconazole ) , which act by inhibiting lanosterol demethylase in the sterol biosynthesis pathway .
	manualset3
178605	1	411109	13	NULL	NULL	0	NULL	reason	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important reason cities continue to exist , given the dramatic drop in transportation costs for physical goods over the last century , is probably related to the forces of agglomeration as they apply to knowledge spillovers .
	manualset3
178606	2	411109	13	NULL	NULL	0	NULL	cities	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important reason cities continue to exist , given the dramatic drop in transportation costs for physical goods over the last century , is probably related to the forces of agglomeration as they apply to knowledge spillovers .
	manualset3
178607	3	411109	13	NULL	NULL	0	NULL	drop	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important reason cities continue to exist , given the dramatic drop in transportation costs for physical goods over the last century , is probably related to the forces of agglomeration as they apply to knowledge spillovers .
	manualset3
178608	4	411109	13	NULL	NULL	0	NULL	transportation costs 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important reason cities continue to exist , given the dramatic drop in transportation costs for physical goods over the last century , is probably related to the forces of agglomeration as they apply to knowledge spillovers .
	manualset3
178609	5	411109	13	NULL	NULL	0	NULL	physical goods 	Thing												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important reason cities continue to exist , given the dramatic drop in transportation costs for physical goods over the last century , is probably related to the forces of agglomeration as they apply to knowledge spillovers .
	manualset3
178610	6	411109	13	NULL	NULL	0	NULL	last century	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important reason cities continue to exist , given the dramatic drop in transportation costs for physical goods over the last century , is probably related to the forces of agglomeration as they apply to knowledge spillovers .
	manualset3
178611	7	411109	13	NULL	NULL	0	NULL	forces 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important reason cities continue to exist , given the dramatic drop in transportation costs for physical goods over the last century , is probably related to the forces of agglomeration as they apply to knowledge spillovers .
	manualset3
178612	8	411109	13	NULL	NULL	0	NULL	agglomeration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important reason cities continue to exist , given the dramatic drop in transportation costs for physical goods over the last century , is probably related to the forces of agglomeration as they apply to knowledge spillovers .
	manualset3
178613	9	411109	13	NULL	NULL	0	NULL	knowledge spillovers	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important reason cities continue to exist , given the dramatic drop in transportation costs for physical goods over the last century , is probably related to the forces of agglomeration as they apply to knowledge spillovers .
	manualset3
178614	1	411110	13	NULL	NULL	0	NULL	reason 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important reason for having childeren was love and care for males , and God 's will for women .
	manualset3
178615	2	411110	13	NULL	NULL	0	NULL	childeren	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important reason for having childeren was love and care for males , and God 's will for women .
	manualset3
178616	3	411110	13	NULL	NULL	0	NULL	love	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important reason for having childeren was love and care for males , and God 's will for women .
	manualset3
178617	4	411110	13	NULL	NULL	0	NULL	care	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important reason for having childeren was love and care for males , and God 's will for women .
	manualset3
178618	5	411110	13	NULL	NULL	0	NULL	males	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important reason for having childeren was love and care for males , and God 's will for women .
	manualset3
178619	6	411110	13	NULL	NULL	0	NULL	God 's will 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important reason for having childeren was love and care for males , and God 's will for women .
	manualset3
178620	7	411110	13	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important reason for having childeren was love and care for males , and God 's will for women .
	manualset3
178621	1	411111	13	NULL	NULL	0	NULL	theoretical aspects	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important theoretical and computational aspects of the coupling between PCM and TDDFT are presented and discussed together with an example of application to the study of the low-lying electronic excited states of push-pull chromophores in different solvents .
	manualset3
178622	2	411111	13	NULL	NULL	0	NULL	computational aspects	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important theoretical and computational aspects of the coupling between PCM and TDDFT are presented and discussed together with an example of application to the study of the low-lying electronic excited states of push-pull chromophores in different solvents .
	manualset3
178623	3	411111	13	NULL	NULL	0	NULL	coupling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important theoretical and computational aspects of the coupling between PCM and TDDFT are presented and discussed together with an example of application to the study of the low-lying electronic excited states of push-pull chromophores in different solvents .
	manualset3
178624	4	411111	13	NULL	NULL	0	NULL	PCM	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important theoretical and computational aspects of the coupling between PCM and TDDFT are presented and discussed together with an example of application to the study of the low-lying electronic excited states of push-pull chromophores in different solvents .
	manualset3
178664	5	411111	13	NULL	NULL	0	NULL	TDDFT	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important theoretical and computational aspects of the coupling between PCM and TDDFT are presented and discussed together with an example of application to the study of the low-lying electronic excited states of push-pull chromophores in different solvents .
	manualset3
178707	6	411111	13	NULL	NULL	0	NULL	example	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important theoretical and computational aspects of the coupling between PCM and TDDFT are presented and discussed together with an example of application to the study of the low-lying electronic excited states of push-pull chromophores in different solvents .
	manualset3
178708	7	411111	13	NULL	NULL	0	NULL	 application 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important theoretical and computational aspects of the coupling between PCM and TDDFT are presented and discussed together with an example of application to the study of the low-lying electronic excited states of push-pull chromophores in different solvents .
	manualset3
178709	8	411111	13	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important theoretical and computational aspects of the coupling between PCM and TDDFT are presented and discussed together with an example of application to the study of the low-lying electronic excited states of push-pull chromophores in different solvents .
	manualset3
178710	9	411111	13	NULL	NULL	0	NULL	low-lying electronic excited states	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important theoretical and computational aspects of the coupling between PCM and TDDFT are presented and discussed together with an example of application to the study of the low-lying electronic excited states of push-pull chromophores in different solvents .
	manualset3
178711	10	411111	13	NULL	NULL	0	NULL	chromophores 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important theoretical and computational aspects of the coupling between PCM and TDDFT are presented and discussed together with an example of application to the study of the low-lying electronic excited states of push-pull chromophores in different solvents .
	manualset3
178712	11	411111	13	NULL	NULL	0	NULL	solvents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important theoretical and computational aspects of the coupling between PCM and TDDFT are presented and discussed together with an example of application to the study of the low-lying electronic excited states of push-pull chromophores in different solvents .
	manualset3
178713	1	411112	13	NULL	NULL	0	NULL	method 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A very controversial method of slaughter .
	manualset3
178714	2	411112	13	NULL	NULL	0	NULL	slaughter	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A very controversial method of slaughter .
	manualset3
178715	1	411113	13	NULL	NULL	0	NULL	explanation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most likely explanation for this finding is aripiprazole 's weak partial agonism at D2-like dopamine receptors .
	manualset3
178716	2	411113	13	NULL	NULL	0	NULL	aripiprazole 's	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The most likely explanation for this finding is aripiprazole 's weak partial agonism at D2-like dopamine receptors .
	manualset3
178717	3	411113	13	NULL	NULL	0	NULL	agonism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The most likely explanation for this finding is aripiprazole 's weak partial agonism at D2-like dopamine receptors .
	manualset3
178718	4	411113	13	NULL	NULL	0	NULL	D2-like dopamine receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The most likely explanation for this finding is aripiprazole 's weak partial agonism at D2-like dopamine receptors .
	manualset3
178720	1	411114	13	NULL	NULL	0	NULL	finding 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most notable finding was that mutations in the same disease gene can be found in different clinical types of cardiomyopathy .
	manualset3
178721	2	411114	13	NULL	NULL	0	NULL	mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The most notable finding was that mutations in the same disease gene can be found in different clinical types of cardiomyopathy .
	manualset3
178722	3	411114	13	NULL	NULL	0	NULL	 disease gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The most notable finding was that mutations in the same disease gene can be found in different clinical types of cardiomyopathy .
	manualset3
178723	4	411114	13	NULL	NULL	0	NULL	clinical types	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most notable finding was that mutations in the same disease gene can be found in different clinical types of cardiomyopathy .
	manualset3
178724	5	411114	13	NULL	NULL	0	NULL	cardiomyopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The most notable finding was that mutations in the same disease gene can be found in different clinical types of cardiomyopathy .
	manualset3
178725	1	411115	13	NULL	NULL	0	NULL	decrease 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most prominent decrease was for CD4 + T cells ( 72-74 % ) , which suggests that a reduction of T cells in the psoriatic plaque might not be a guarantee for positive clinical outcomes .
	manualset3
178726	2	411115	13	NULL	NULL	0	NULL	CD4 + T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The most prominent decrease was for CD4 + T cells ( 72-74 % ) , which suggests that a reduction of T cells in the psoriatic plaque might not be a guarantee for positive clinical outcomes .
	manualset3
178727	3	411115	13	NULL	NULL	0	NULL	72-74 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The most prominent decrease was for CD4 + T cells ( 72-74 % ) , which suggests that a reduction of T cells in the psoriatic plaque might not be a guarantee for positive clinical outcomes .
	manualset3
178728	4	411115	13	NULL	NULL	0	NULL	reduction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most prominent decrease was for CD4 + T cells ( 72-74 % ) , which suggests that a reduction of T cells in the psoriatic plaque might not be a guarantee for positive clinical outcomes .
	manualset3
178729	5	411115	13	NULL	NULL	0	NULL	T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The most prominent decrease was for CD4 + T cells ( 72-74 % ) , which suggests that a reduction of T cells in the psoriatic plaque might not be a guarantee for positive clinical outcomes .
	manualset3
178730	6	411115	13	NULL	NULL	0	NULL	psoriatic plaque	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most prominent decrease was for CD4 + T cells ( 72-74 % ) , which suggests that a reduction of T cells in the psoriatic plaque might not be a guarantee for positive clinical outcomes .
	manualset3
178732	7	411115	13	NULL	NULL	0	NULL	guarantee	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most prominent decrease was for CD4 + T cells ( 72-74 % ) , which suggests that a reduction of T cells in the psoriatic plaque might not be a guarantee for positive clinical outcomes .
	manualset3
178733	8	411115	13	NULL	NULL	0	NULL	positive clinical outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most prominent decrease was for CD4 + T cells ( 72-74 % ) , which suggests that a reduction of T cells in the psoriatic plaque might not be a guarantee for positive clinical outcomes .
	manualset3
178756	1	411116	13	NULL	NULL	0	NULL	proton pump inhibitor	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The most recently developed proton pump inhibitor , lansoprazole , at doses of 15 , 30 , or 60 mg/day for 4 and 8 weeks of treatment , has proven to be significantly more effective than placebo ( one multicenter study involving 292 patients ) or ranitidine ( three multicenter studies involving 653 patients ) in terms of mucosal healing and symptom relief .
	manualset3
178757	2	411116	13	NULL	NULL	0	NULL	lansoprazole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The most recently developed proton pump inhibitor , lansoprazole , at doses of 15 , 30 , or 60 mg/day for 4 and 8 weeks of treatment , has proven to be significantly more effective than placebo ( one multicenter study involving 292 patients ) or ranitidine ( three multicenter studies involving 653 patients ) in terms of mucosal healing and symptom relief .
	manualset3
178760	3	411116	13	NULL	NULL	0	NULL	doses of 15 mg/day	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The most recently developed proton pump inhibitor , lansoprazole , at doses of 15 , 30 , or 60 mg/day for 4 and 8 weeks of treatment , has proven to be significantly more effective than placebo ( one multicenter study involving 292 patients ) or ranitidine ( three multicenter studies involving 653 patients ) in terms of mucosal healing and symptom relief .
	manualset3
178761	4	411116	13	NULL	NULL	NULL	NULL	doses of 30 mg/day	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The most recently developed proton pump inhibitor , lansoprazole , at doses of 15 , 30 , or 60 mg/day for 4 and 8 weeks of treatment , has proven to be significantly more effective than placebo ( one multicenter study involving 292 patients ) or ranitidine ( three multicenter studies involving 653 patients ) in terms of mucosal healing and symptom relief .
	manualset3
178762	5	411116	13	NULL	NULL	NULL	NULL	doses of 60 mg/day	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The most recently developed proton pump inhibitor , lansoprazole , at doses of 15 , 30 , or 60 mg/day for 4 and 8 weeks of treatment , has proven to be significantly more effective than placebo ( one multicenter study involving 292 patients ) or ranitidine ( three multicenter studies involving 653 patients ) in terms of mucosal healing and symptom relief .
	manualset3
178763	6	411116	13	NULL	NULL	0	NULL	4 weeks 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The most recently developed proton pump inhibitor , lansoprazole , at doses of 15 , 30 , or 60 mg/day for 4 and 8 weeks of treatment , has proven to be significantly more effective than placebo ( one multicenter study involving 292 patients ) or ranitidine ( three multicenter studies involving 653 patients ) in terms of mucosal healing and symptom relief .
	manualset3
178764	7	411116	13	NULL	NULL	0	NULL	8 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The most recently developed proton pump inhibitor , lansoprazole , at doses of 15 , 30 , or 60 mg/day for 4 and 8 weeks of treatment , has proven to be significantly more effective than placebo ( one multicenter study involving 292 patients ) or ranitidine ( three multicenter studies involving 653 patients ) in terms of mucosal healing and symptom relief .
	manualset3
178765	8	411116	13	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The most recently developed proton pump inhibitor , lansoprazole , at doses of 15 , 30 , or 60 mg/day for 4 and 8 weeks of treatment , has proven to be significantly more effective than placebo ( one multicenter study involving 292 patients ) or ranitidine ( three multicenter studies involving 653 patients ) in terms of mucosal healing and symptom relief .
	manualset3
178766	9	411116	13	NULL	NULL	0	NULL	placebo	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The most recently developed proton pump inhibitor , lansoprazole , at doses of 15 , 30 , or 60 mg/day for 4 and 8 weeks of treatment , has proven to be significantly more effective than placebo ( one multicenter study involving 292 patients ) or ranitidine ( three multicenter studies involving 653 patients ) in terms of mucosal healing and symptom relief .
	manualset3
178767	10	411116	13	NULL	NULL	0	NULL	multicenter study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The most recently developed proton pump inhibitor , lansoprazole , at doses of 15 , 30 , or 60 mg/day for 4 and 8 weeks of treatment , has proven to be significantly more effective than placebo ( one multicenter study involving 292 patients ) or ranitidine ( three multicenter studies involving 653 patients ) in terms of mucosal healing and symptom relief .
	manualset3
178768	11	411116	13	NULL	NULL	0	NULL	292 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The most recently developed proton pump inhibitor , lansoprazole , at doses of 15 , 30 , or 60 mg/day for 4 and 8 weeks of treatment , has proven to be significantly more effective than placebo ( one multicenter study involving 292 patients ) or ranitidine ( three multicenter studies involving 653 patients ) in terms of mucosal healing and symptom relief .
	manualset3
178769	12	411116	13	NULL	NULL	0	NULL	ranitidine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The most recently developed proton pump inhibitor , lansoprazole , at doses of 15 , 30 , or 60 mg/day for 4 and 8 weeks of treatment , has proven to be significantly more effective than placebo ( one multicenter study involving 292 patients ) or ranitidine ( three multicenter studies involving 653 patients ) in terms of mucosal healing and symptom relief .
	manualset3
178770	13	411116	13	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The most recently developed proton pump inhibitor , lansoprazole , at doses of 15 , 30 , or 60 mg/day for 4 and 8 weeks of treatment , has proven to be significantly more effective than placebo ( one multicenter study involving 292 patients ) or ranitidine ( three multicenter studies involving 653 patients ) in terms of mucosal healing and symptom relief .
	manualset3
178771	14	411116	13	NULL	NULL	0	NULL	multicenter studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The most recently developed proton pump inhibitor , lansoprazole , at doses of 15 , 30 , or 60 mg/day for 4 and 8 weeks of treatment , has proven to be significantly more effective than placebo ( one multicenter study involving 292 patients ) or ranitidine ( three multicenter studies involving 653 patients ) in terms of mucosal healing and symptom relief .
	manualset3
178772	15	411116	13	NULL	NULL	0	NULL	653 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The most recently developed proton pump inhibitor , lansoprazole , at doses of 15 , 30 , or 60 mg/day for 4 and 8 weeks of treatment , has proven to be significantly more effective than placebo ( one multicenter study involving 292 patients ) or ranitidine ( three multicenter studies involving 653 patients ) in terms of mucosal healing and symptom relief .
	manualset3
178773	16	411116	13	NULL	NULL	0	NULL	terms 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most recently developed proton pump inhibitor , lansoprazole , at doses of 15 , 30 , or 60 mg/day for 4 and 8 weeks of treatment , has proven to be significantly more effective than placebo ( one multicenter study involving 292 patients ) or ranitidine ( three multicenter studies involving 653 patients ) in terms of mucosal healing and symptom relief .
	manualset3
178774	17	411116	13	NULL	NULL	0	NULL	mucosal healing 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most recently developed proton pump inhibitor , lansoprazole , at doses of 15 , 30 , or 60 mg/day for 4 and 8 weeks of treatment , has proven to be significantly more effective than placebo ( one multicenter study involving 292 patients ) or ranitidine ( three multicenter studies involving 653 patients ) in terms of mucosal healing and symptom relief .
	manualset3
178775	18	411116	13	NULL	NULL	0	NULL	symptom relief	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most recently developed proton pump inhibitor , lansoprazole , at doses of 15 , 30 , or 60 mg/day for 4 and 8 weeks of treatment , has proven to be significantly more effective than placebo ( one multicenter study involving 292 patients ) or ranitidine ( three multicenter studies involving 653 patients ) in terms of mucosal healing and symptom relief .
	manualset3
178776	1	411117	13	NULL	NULL	0	NULL	responsive cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The most responsive cell observed thus far is the CCL64 mink lung cell line .
	manualset3
178777	2	411117	13	NULL	NULL	0	NULL	CCL64 mink lung cell line 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The most responsive cell observed thus far is the CCL64 mink lung cell line .
	manualset3
178778	1	411118	13	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A very high correlation was found between the assessment of knee skeletal ages by the RWT method and that of the hand-wrist by the GP and TW2 systems in the same subject without sex and age-associated variations .
	manualset3
178779	2	411118	13	NULL	NULL	0	NULL	assessment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A very high correlation was found between the assessment of knee skeletal ages by the RWT method and that of the hand-wrist by the GP and TW2 systems in the same subject without sex and age-associated variations .
	manualset3
178780	3	411118	13	NULL	NULL	0	NULL	knee skeletal ages	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A very high correlation was found between the assessment of knee skeletal ages by the RWT method and that of the hand-wrist by the GP and TW2 systems in the same subject without sex and age-associated variations .
	manualset3
178781	4	411118	13	NULL	NULL	0	NULL	RWT method 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A very high correlation was found between the assessment of knee skeletal ages by the RWT method and that of the hand-wrist by the GP and TW2 systems in the same subject without sex and age-associated variations .
	manualset3
178782	5	411118	13	NULL	NULL	0	NULL	hand-wrist	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A very high correlation was found between the assessment of knee skeletal ages by the RWT method and that of the hand-wrist by the GP and TW2 systems in the same subject without sex and age-associated variations .
	manualset3
178783	6	411118	13	NULL	NULL	0	NULL	GP system	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A very high correlation was found between the assessment of knee skeletal ages by the RWT method and that of the hand-wrist by the GP and TW2 systems in the same subject without sex and age-associated variations .
	manualset3
178784	7	411118	13	NULL	NULL	0	NULL	TW2 system	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A very high correlation was found between the assessment of knee skeletal ages by the RWT method and that of the hand-wrist by the GP and TW2 systems in the same subject without sex and age-associated variations .
	manualset3
178785	8	411118	13	NULL	NULL	0	NULL	subject	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A very high correlation was found between the assessment of knee skeletal ages by the RWT method and that of the hand-wrist by the GP and TW2 systems in the same subject without sex and age-associated variations .
	manualset3
178786	9	411118	13	NULL	NULL	0	NULL	sex variations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A very high correlation was found between the assessment of knee skeletal ages by the RWT method and that of the hand-wrist by the GP and TW2 systems in the same subject without sex and age-associated variations .
	manualset3
178787	10	411118	13	NULL	NULL	0	NULL	age-associated variations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A very high correlation was found between the assessment of knee skeletal ages by the RWT method and that of the hand-wrist by the GP and TW2 systems in the same subject without sex and age-associated variations .
	manualset3
178788	1	411119	13	NULL	NULL	0	NULL	ultrastructural feature 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The most striking ultrastructural feature of these AM was the abundance of finger-like microvilli on the cell surface before phagocytosis ; after ingestion of SRBC into phagocytic vacuoles there were only a few short microvilli on the surface .
	manualset3
178789	2	411119	13	NULL	NULL	0	NULL	AM	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The most striking ultrastructural feature of these AM was the abundance of finger-like microvilli on the cell surface before phagocytosis ; after ingestion of SRBC into phagocytic vacuoles there were only a few short microvilli on the surface .
	manualset3
178790	3	411119	13	NULL	NULL	0	NULL	abundance	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The most striking ultrastructural feature of these AM was the abundance of finger-like microvilli on the cell surface before phagocytosis ; after ingestion of SRBC into phagocytic vacuoles there were only a few short microvilli on the surface .
	manualset3
178791	4	411119	13	NULL	NULL	0	NULL	finger-like microvilli 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The most striking ultrastructural feature of these AM was the abundance of finger-like microvilli on the cell surface before phagocytosis ; after ingestion of SRBC into phagocytic vacuoles there were only a few short microvilli on the surface .
	manualset3
178792	5	411119	13	NULL	NULL	0	NULL	cell surface 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The most striking ultrastructural feature of these AM was the abundance of finger-like microvilli on the cell surface before phagocytosis ; after ingestion of SRBC into phagocytic vacuoles there were only a few short microvilli on the surface .
	manualset3
178793	6	411119	13	NULL	NULL	0	NULL	phagocytosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The most striking ultrastructural feature of these AM was the abundance of finger-like microvilli on the cell surface before phagocytosis ; after ingestion of SRBC into phagocytic vacuoles there were only a few short microvilli on the surface .
	manualset3
178794	7	411119	13	NULL	NULL	0	NULL	ingestion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most striking ultrastructural feature of these AM was the abundance of finger-like microvilli on the cell surface before phagocytosis ; after ingestion of SRBC into phagocytic vacuoles there were only a few short microvilli on the surface .
	manualset3
178795	8	411119	13	NULL	NULL	0	NULL	SRBC 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The most striking ultrastructural feature of these AM was the abundance of finger-like microvilli on the cell surface before phagocytosis ; after ingestion of SRBC into phagocytic vacuoles there were only a few short microvilli on the surface .
	manualset3
178796	9	411119	13	NULL	NULL	0	NULL	phagocytic vacuoles 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The most striking ultrastructural feature of these AM was the abundance of finger-like microvilli on the cell surface before phagocytosis ; after ingestion of SRBC into phagocytic vacuoles there were only a few short microvilli on the surface .
	manualset3
178797	10	411119	13	NULL	NULL	0	NULL	short microvilli	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The most striking ultrastructural feature of these AM was the abundance of finger-like microvilli on the cell surface before phagocytosis ; after ingestion of SRBC into phagocytic vacuoles there were only a few short microvilli on the surface .
	manualset3
178798	11	411119	13	NULL	NULL	0	NULL	surface	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The most striking ultrastructural feature of these AM was the abundance of finger-like microvilli on the cell surface before phagocytosis ; after ingestion of SRBC into phagocytic vacuoles there were only a few short microvilli on the surface .
	manualset3
178799	1	411120	13	NULL	NULL	0	NULL	group of T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The most studied group of T cells that interact with lipid antigens are natural killer T ( NKT ) cells , which characteristically express a semi-invariant T-cell receptor ( NKT TCR ) that specifically recognizes the CD1 family member , CD1d .
	manualset3
178800	2	411120	13	NULL	NULL	0	NULL	lipid antigens	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The most studied group of T cells that interact with lipid antigens are natural killer T ( NKT ) cells , which characteristically express a semi-invariant T-cell receptor ( NKT TCR ) that specifically recognizes the CD1 family member , CD1d .
	manualset3
178801	3	411120	13	NULL	NULL	0	NULL	natural killer T ( NKT ) cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The most studied group of T cells that interact with lipid antigens are natural killer T ( NKT ) cells , which characteristically express a semi-invariant T-cell receptor ( NKT TCR ) that specifically recognizes the CD1 family member , CD1d .
	manualset3
178802	4	411120	13	NULL	NULL	0	NULL	semi-invariant T-cell receptor ( NKT TCR ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The most studied group of T cells that interact with lipid antigens are natural killer T ( NKT ) cells , which characteristically express a semi-invariant T-cell receptor ( NKT TCR ) that specifically recognizes the CD1 family member , CD1d .
	manualset3
178803	5	411120	13	NULL	NULL	0	NULL	CD1 family member	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The most studied group of T cells that interact with lipid antigens are natural killer T ( NKT ) cells , which characteristically express a semi-invariant T-cell receptor ( NKT TCR ) that specifically recognizes the CD1 family member , CD1d .
	manualset3
178804	6	411120	13	NULL	NULL	0	NULL	CD1d 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The most studied group of T cells that interact with lipid antigens are natural killer T ( NKT ) cells , which characteristically express a semi-invariant T-cell receptor ( NKT TCR ) that specifically recognizes the CD1 family member , CD1d .
	manualset3
178805	1	411121	13	NULL	NULL	0	NULL	mother 's 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The mother 's calcium , phosphorus , and alkaline phosphatase levels were normal .
	manualset3
178806	2	411121	13	NULL	NULL	0	NULL	calcium levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The mother 's calcium , phosphorus , and alkaline phosphatase levels were normal .
	manualset3
178807	3	411121	13	NULL	NULL	0	NULL	phosphorus levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The mother 's calcium , phosphorus , and alkaline phosphatase levels were normal .
	manualset3
178808	4	411121	13	NULL	NULL	0	NULL	alkaline phosphatase levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The mother 's calcium , phosphorus , and alkaline phosphatase levels were normal .
	manualset3
178809	1	411122	13	NULL	NULL	0	NULL	motif	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The motif belongs to a Plasmodium falciparum malarial peptide coded 1513 , derived from the MSP-1 protein .
	manualset3
178810	2	411122	13	NULL	NULL	0	NULL	Plasmodium falciparum malarial peptide coded 1513	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The motif belongs to a Plasmodium falciparum malarial peptide coded 1513 , derived from the MSP-1 protein .
	manualset3
178811	3	411122	13	NULL	NULL	0	NULL	MSP-1 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The motif belongs to a Plasmodium falciparum malarial peptide coded 1513 , derived from the MSP-1 protein .
	manualset3
178812	1	411123	13	NULL	NULL	0	NULL	motor nerve conduction velocity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The motor nerve conduction velocity improved by at least 10 % in one ulnar nerve in seven patients and worsened in two .
	manualset3
178813	2	411123	13	NULL	NULL	0	NULL	10 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The motor nerve conduction velocity improved by at least 10 % in one ulnar nerve in seven patients and worsened in two .
	manualset3
178814	3	411123	13	NULL	NULL	0	NULL	ulnar nerve	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The motor nerve conduction velocity improved by at least 10 % in one ulnar nerve in seven patients and worsened in two .
	manualset3
178815	4	411123	13	NULL	NULL	0	NULL	seven patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The motor nerve conduction velocity improved by at least 10 % in one ulnar nerve in seven patients and worsened in two .
	manualset3
178816	5	411123	13	NULL	NULL	0	NULL	two 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The motor nerve conduction velocity improved by at least 10 % in one ulnar nerve in seven patients and worsened in two .
	manualset3
178817	1	411124	13	NULL	NULL	0	NULL	mouse	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The mouse also shows distinct profiles generated by differential expression levels of the SMRT transcript isoforms .
	manualset3
178818	2	411124	13	NULL	NULL	0	NULL	profiles	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The mouse also shows distinct profiles generated by differential expression levels of the SMRT transcript isoforms .
	manualset3
178819	3	411124	13	NULL	NULL	0	NULL	expression levels 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The mouse also shows distinct profiles generated by differential expression levels of the SMRT transcript isoforms .
	manualset3
178820	4	411124	13	NULL	NULL	0	NULL	SMRT transcript isoforms	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The mouse also shows distinct profiles generated by differential expression levels of the SMRT transcript isoforms .
	manualset3
178821	1	411125	13	NULL	NULL	0	NULL	mouse genome 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The mouse genome contains one TRiC5 gene and one TRiC5 pseudogene located on chromosomes 3F and 5B , respectively .
	manualset3
178822	2	411125	13	NULL	NULL	0	NULL	TRiC5 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The mouse genome contains one TRiC5 gene and one TRiC5 pseudogene located on chromosomes 3F and 5B , respectively .
	manualset3
178823	3	411125	13	NULL	NULL	0	NULL	TRiC5 pseudogene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The mouse genome contains one TRiC5 gene and one TRiC5 pseudogene located on chromosomes 3F and 5B , respectively .
	manualset3
178824	4	411125	13	NULL	NULL	0	NULL	chromosomes 3F	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The mouse genome contains one TRiC5 gene and one TRiC5 pseudogene located on chromosomes 3F and 5B , respectively .
	manualset3
178825	5	411125	13	NULL	NULL	0	NULL	chromosomes 5B	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The mouse genome contains one TRiC5 gene and one TRiC5 pseudogene located on chromosomes 3F and 5B , respectively .
	manualset3
178826	1	411126	13	NULL	NULL	0	NULL	Clinical experience	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical experience with synthetic penicillin preparation ( Broadcillin ` Banyu ' ) ) .
	manualset3
178827	2	411126	13	NULL	NULL	0	NULL	synthetic penicillin preparation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical experience with synthetic penicillin preparation ( Broadcillin ` Banyu ' ) ) .
	manualset3
178828	3	411126	13	NULL	NULL	0	NULL	Broadcillin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical experience with synthetic penicillin preparation ( Broadcillin ` Banyu ' ) ) .
	manualset3
178829	4	411126	13	NULL	NULL	0	NULL	Banyu 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical experience with synthetic penicillin preparation ( Broadcillin ` Banyu ' ) ) .
	manualset3
178830	1	411127	13	NULL	NULL	0	NULL	section	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A very important section is devoted to eye-to-hand coordination .
	manualset3
178831	2	411127	13	NULL	NULL	0	NULL	eye-to-hand coordination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A very important section is devoted to eye-to-hand coordination .
	manualset3
178832	1	411128	13	NULL	NULL	0	NULL	mucin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mucin could not be found in mouse serum samples taken before day 46 .
	manualset3
178833	2	411128	13	NULL	NULL	0	NULL	mouse serum samples 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The mucin could not be found in mouse serum samples taken before day 46 .
	manualset3
178834	3	411128	13	NULL	NULL	0	NULL	day 46	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The mucin could not be found in mouse serum samples taken before day 46 .
	manualset3
178835	1	411129	13	NULL	NULL	0	NULL	multidrug resistance protein P-glycoprotein ( P-gp ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The multidrug resistance protein P-glycoprotein ( P-gp ) is physiologically expressed at the bile canalicular membrane of the liver , where it participates in the biliary excretion of various lipophilic drugs .
	manualset3
178836	2	411129	13	NULL	NULL	0	NULL	bile canalicular membrane	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The multidrug resistance protein P-glycoprotein ( P-gp ) is physiologically expressed at the bile canalicular membrane of the liver , where it participates in the biliary excretion of various lipophilic drugs .
	manualset3
178837	3	411129	13	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The multidrug resistance protein P-glycoprotein ( P-gp ) is physiologically expressed at the bile canalicular membrane of the liver , where it participates in the biliary excretion of various lipophilic drugs .
	manualset3
178838	4	411129	13	NULL	NULL	0	NULL	biliary excretion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The multidrug resistance protein P-glycoprotein ( P-gp ) is physiologically expressed at the bile canalicular membrane of the liver , where it participates in the biliary excretion of various lipophilic drugs .
	manualset3
178839	5	411129	13	NULL	NULL	0	NULL	lipophilic drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The multidrug resistance protein P-glycoprotein ( P-gp ) is physiologically expressed at the bile canalicular membrane of the liver , where it participates in the biliary excretion of various lipophilic drugs .
	manualset3
178840	1	411130	13	NULL	NULL	NULL	NULL	 multifunctional DNA repair 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The multifunctional DNA repair/redox enzyme Ape1/Ref -1 promotes survival of neurons after oxidative stress .
	manualset3
178841	2	411130	13	NULL	NULL	0	NULL	survival 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The multifunctional DNA repair/redox enzyme Ape1/Ref -1 promotes survival of neurons after oxidative stress .
	manualset3
178842	3	411130	13	NULL	NULL	0	NULL	neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The multifunctional DNA repair/redox enzyme Ape1/Ref -1 promotes survival of neurons after oxidative stress .
	manualset3
178843	4	411130	13	NULL	NULL	NULL	NULL	oxidative stress	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The multifunctional DNA repair/redox enzyme Ape1/Ref -1 promotes survival of neurons after oxidative stress .
	manualset3
178936	5	411130	13	NULL	NULL	0	NULL	redox enzyme Ape1/Ref -1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The multifunctional DNA repair/redox enzyme Ape1/Ref -1 promotes survival of neurons after oxidative stress .
	manualset3
157831	1	411331	7	NULL	NULL	0	NULL	organism	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The organism exhibited in vitro heteroresistance to daptomycin , with two subpopulations showing daptomycin susceptibility ( MIC of 0.094 g/ml ) and high-level resistance to daptomycin ( MIC of 256 g/ml ) .
	manualset3
157833	3	411331	7	NULL	NULL	0	NULL	daptomycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The organism exhibited in vitro heteroresistance to daptomycin , with two subpopulations showing daptomycin susceptibility ( MIC of 0.094 g/ml ) and high-level resistance to daptomycin ( MIC of 256 g/ml ) .
	manualset3
157834	5	411331	7	NULL	NULL	NULL	NULL	daptomycin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The organism exhibited in vitro heteroresistance to daptomycin , with two subpopulations showing daptomycin susceptibility ( MIC of 0.094 g/ml ) and high-level resistance to daptomycin ( MIC of 256 g/ml ) .
	manualset3
157835	6	411331	7	NULL	NULL	NULL	NULL	MIC of 0.094 g/ml 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The organism exhibited in vitro heteroresistance to daptomycin , with two subpopulations showing daptomycin susceptibility ( MIC of 0.094 g/ml ) and high-level resistance to daptomycin ( MIC of 256 g/ml ) .
	manualset3
157837	7	411331	7	NULL	NULL	NULL	NULL	high-level resistance	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The organism exhibited in vitro heteroresistance to daptomycin , with two subpopulations showing daptomycin susceptibility ( MIC of 0.094 g/ml ) and high-level resistance to daptomycin ( MIC of 256 g/ml ) .
	manualset3
157838	8	411331	7	NULL	NULL	0	NULL	daptomycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The organism exhibited in vitro heteroresistance to daptomycin , with two subpopulations showing daptomycin susceptibility ( MIC of 0.094 g/ml ) and high-level resistance to daptomycin ( MIC of 256 g/ml ) .
	manualset3
157839	9	411331	7	NULL	NULL	NULL	NULL	MIC of 256 g/ml	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The organism exhibited in vitro heteroresistance to daptomycin , with two subpopulations showing daptomycin susceptibility ( MIC of 0.094 g/ml ) and high-level resistance to daptomycin ( MIC of 256 g/ml ) .
	manualset3
157841	4	411331	7	NULL	NULL	NULL	NULL	subpopulations	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The organism exhibited in vitro heteroresistance to daptomycin , with two subpopulations showing daptomycin susceptibility ( MIC of 0.094 g/ml ) and high-level resistance to daptomycin ( MIC of 256 g/ml ) .
	manualset3
158512	11	411331	7	NULL	NULL	NULL	NULL	heteroresistance	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The organism exhibited in vitro heteroresistance to daptomycin , with two subpopulations showing daptomycin susceptibility ( MIC of 0.094 g/ml ) and high-level resistance to daptomycin ( MIC of 256 g/ml ) .
	manualset3
158513	10	411331	7	NULL	NULL	NULL	NULL	susceptibility	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The organism exhibited in vitro heteroresistance to daptomycin , with two subpopulations showing daptomycin susceptibility ( MIC of 0.094 g/ml ) and high-level resistance to daptomycin ( MIC of 256 g/ml ) .
	manualset3
157842	1	411332	7	NULL	NULL	0	NULL	organism	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The organism possesses a complex branched respiratory chain that has the ability to utilize different electron donors .
	manualset3
157843	2	411332	7	NULL	NULL	0	NULL	complex branched respiratory chain	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The organism possesses a complex branched respiratory chain that has the ability to utilize different electron donors .
	manualset3
157844	3	411332	7	NULL	NULL	0	NULL	electron donors	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The organism possesses a complex branched respiratory chain that has the ability to utilize different electron donors .
	manualset3
157845	1	411333	7	NULL	NULL	0	NULL	origin of lipids	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The origin and distribution of lipids in aortic atherosclerosis .
	manualset3
157846	2	411333	7	NULL	NULL	0	NULL	 distribution of lipids	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The origin and distribution of lipids in aortic atherosclerosis .
	manualset3
157847	3	411333	7	NULL	NULL	0	NULL	aortic atherosclerosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The origin and distribution of lipids in aortic atherosclerosis .
	manualset3
157848	1	411334	7	NULL	NULL	NULL	NULL	origin of waves	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The origin and propagation of waves of spontaneous excitation in bundles of smooth muscle of the guinea-pig bladder were examined using intracellular recording techniques and visualization of the changes in the intracellular calcium concentration ( ( Ca2 + ) i ) .
	manualset3
157849	2	411334	7	NULL	NULL	NULL	NULL	propagation of waves	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The origin and propagation of waves of spontaneous excitation in bundles of smooth muscle of the guinea-pig bladder were examined using intracellular recording techniques and visualization of the changes in the intracellular calcium concentration ( ( Ca2 + ) i ) .
	manualset3
157850	3	411334	7	NULL	NULL	0	NULL	spontaneous excitation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The origin and propagation of waves of spontaneous excitation in bundles of smooth muscle of the guinea-pig bladder were examined using intracellular recording techniques and visualization of the changes in the intracellular calcium concentration ( ( Ca2 + ) i ) .
	manualset3
157851	4	411334	7	NULL	NULL	0	NULL	bundles of smooth muscle 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The origin and propagation of waves of spontaneous excitation in bundles of smooth muscle of the guinea-pig bladder were examined using intracellular recording techniques and visualization of the changes in the intracellular calcium concentration ( ( Ca2 + ) i ) .
	manualset3
157852	5	411334	7	NULL	NULL	0	NULL	guinea-pig bladder	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The origin and propagation of waves of spontaneous excitation in bundles of smooth muscle of the guinea-pig bladder were examined using intracellular recording techniques and visualization of the changes in the intracellular calcium concentration ( ( Ca2 + ) i ) .
	manualset3
157853	6	411334	7	NULL	NULL	0	NULL	intracellular recording techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The origin and propagation of waves of spontaneous excitation in bundles of smooth muscle of the guinea-pig bladder were examined using intracellular recording techniques and visualization of the changes in the intracellular calcium concentration ( ( Ca2 + ) i ) .
	manualset3
157854	7	411334	7	NULL	NULL	0	NULL	visualization 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The origin and propagation of waves of spontaneous excitation in bundles of smooth muscle of the guinea-pig bladder were examined using intracellular recording techniques and visualization of the changes in the intracellular calcium concentration ( ( Ca2 + ) i ) .
	manualset3
157855	8	411334	7	NULL	NULL	0	NULL	intracellular calcium concentration ( ( Ca2 + ) i )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The origin and propagation of waves of spontaneous excitation in bundles of smooth muscle of the guinea-pig bladder were examined using intracellular recording techniques and visualization of the changes in the intracellular calcium concentration ( ( Ca2 + ) i ) .
	manualset3
161001	9	411334	7	NULL	NULL	0	NULL	changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The origin and propagation of waves of spontaneous excitation in bundles of smooth muscle of the guinea-pig bladder were examined using intracellular recording techniques and visualization of the changes in the intracellular calcium concentration ( ( Ca2 + ) i ) .
	manualset3
157856	1	411335	7	NULL	NULL	NULL	NULL	ACL forces	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ACL forces dropped to zero during the swing phase in all trials .
	manualset3
157857	2	411335	7	NULL	NULL	0	NULL	 zero 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	ACL forces dropped to zero during the swing phase in all trials .
	manualset3
157858	3	411335	7	NULL	NULL	NULL	NULL	swing phase	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ACL forces dropped to zero during the swing phase in all trials .
	manualset3
157859	4	411335	7	NULL	NULL	0	NULL	trials	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	ACL forces dropped to zero during the swing phase in all trials .
	manualset3
157860	1	411336	7	NULL	NULL	0	NULL	origin of PACAP-IR nerve fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The origin of PACAP-IR nerve fibers which innervate mucous glands and blood vessels may be the autonomic ganglion .
	manualset3
157861	2	411336	7	NULL	NULL	0	NULL	mucous glands	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The origin of PACAP-IR nerve fibers which innervate mucous glands and blood vessels may be the autonomic ganglion .
	manualset3
157862	3	411336	7	NULL	NULL	0	NULL	blood vessels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The origin of PACAP-IR nerve fibers which innervate mucous glands and blood vessels may be the autonomic ganglion .
	manualset3
157863	4	411336	7	NULL	NULL	0	NULL	autonomic ganglion	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The origin of PACAP-IR nerve fibers which innervate mucous glands and blood vessels may be the autonomic ganglion .
	manualset3
157864	5	411336	7	NULL	NULL	0	NULL	innervate 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The origin of PACAP-IR nerve fibers which innervate mucous glands and blood vessels may be the autonomic ganglion .
	manualset3
157865	1	411337	7	NULL	NULL	0	NULL	origin of the KIE	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The origin of the KIE is related to a high propensity for transition state recrossing in this system , with heavier masses recrossing less .
	manualset3
157866	2	411337	7	NULL	NULL	NULL	NULL	high propensity	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The origin of the KIE is related to a high propensity for transition state recrossing in this system , with heavier masses recrossing less .
	manualset3
157867	3	411337	7	NULL	NULL	0	NULL	transition state	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The origin of the KIE is related to a high propensity for transition state recrossing in this system , with heavier masses recrossing less .
	manualset3
157868	4	411337	7	NULL	NULL	NULL	NULL	system	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The origin of the KIE is related to a high propensity for transition state recrossing in this system , with heavier masses recrossing less .
	manualset3
161002	5	411337	7	NULL	NULL	0	NULL	masses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The origin of the KIE is related to a high propensity for transition state recrossing in this system , with heavier masses recrossing less .
	manualset3
157869	1	411338	7	NULL	NULL	NULL	NULL	 origins of the cancers 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The origins of the cancers were the breast ( five patients ) , ovary ( three ) , endometrium ( one ) , and fallopian tube ( one ) .
	manualset3
157870	2	411338	7	NULL	NULL	0	NULL	breast	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The origins of the cancers were the breast ( five patients ) , ovary ( three ) , endometrium ( one ) , and fallopian tube ( one ) .
	manualset3
157871	3	411338	7	NULL	NULL	0	NULL	 five patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The origins of the cancers were the breast ( five patients ) , ovary ( three ) , endometrium ( one ) , and fallopian tube ( one ) .
	manualset3
157872	4	411338	7	NULL	NULL	0	NULL	ovary	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The origins of the cancers were the breast ( five patients ) , ovary ( three ) , endometrium ( one ) , and fallopian tube ( one ) .
	manualset3
157873	5	411338	7	NULL	NULL	0	NULL	three	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The origins of the cancers were the breast ( five patients ) , ovary ( three ) , endometrium ( one ) , and fallopian tube ( one ) .
	manualset3
157874	6	411338	7	NULL	NULL	0	NULL	endometrium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The origins of the cancers were the breast ( five patients ) , ovary ( three ) , endometrium ( one ) , and fallopian tube ( one ) .
	manualset3
157875	7	411338	7	NULL	NULL	0	NULL	one	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The origins of the cancers were the breast ( five patients ) , ovary ( three ) , endometrium ( one ) , and fallopian tube ( one ) .
	manualset3
157876	8	411338	7	NULL	NULL	0	NULL	 fallopian tube	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The origins of the cancers were the breast ( five patients ) , ovary ( three ) , endometrium ( one ) , and fallopian tube ( one ) .
	manualset3
157877	9	411338	7	NULL	NULL	0	NULL	one	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The origins of the cancers were the breast ( five patients ) , ovary ( three ) , endometrium ( one ) , and fallopian tube ( one ) .
	manualset3
157878	1	411339	7	NULL	NULL	0	NULL	oscillatory forces	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The oscillatory forces of nanoparticle suspensions with a particle diameter of 26 nm are measured by a colloidal-probe atomic force microscope ( CP-AFM ) .
	manualset3
157879	2	411339	7	NULL	NULL	NULL	NULL	nanoparticle suspensions	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The oscillatory forces of nanoparticle suspensions with a particle diameter of 26 nm are measured by a colloidal-probe atomic force microscope ( CP-AFM ) .
	manualset3
157880	3	411339	7	NULL	NULL	0	NULL	 particle diameter of 26 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The oscillatory forces of nanoparticle suspensions with a particle diameter of 26 nm are measured by a colloidal-probe atomic force microscope ( CP-AFM ) .
	manualset3
157881	4	411339	7	NULL	NULL	0	NULL	colloidal-probe atomic force microscope ( CP-AFM )	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The oscillatory forces of nanoparticle suspensions with a particle diameter of 26 nm are measured by a colloidal-probe atomic force microscope ( CP-AFM ) .
	manualset3
157882	1	411340	7	NULL	NULL	NULL	NULL	osmotic fragility	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The osmotic fragility was measured using a coil planet centrifuge ( CPC ) system .
	manualset3
157883	2	411340	7	NULL	NULL	0	NULL	coil planet centrifuge ( CPC ) system	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The osmotic fragility was measured using a coil planet centrifuge ( CPC ) system .
	manualset3
157884	1	411341	7	NULL	NULL	0	NULL	carotenoid producing species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The other carotenoid producing species Cystofilobasidium capitatum , Sporobolomyces salmonicolor , and S. roseus were active only against about 40 % of the tested strains and exhibited weak activity .
	manualset3
157885	2	411341	7	NULL	NULL	0	NULL	Cystofilobasidium capitatum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The other carotenoid producing species Cystofilobasidium capitatum , Sporobolomyces salmonicolor , and S. roseus were active only against about 40 % of the tested strains and exhibited weak activity .
	manualset3
157886	3	411341	7	NULL	NULL	0	NULL	Sporobolomyces salmonicolor	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The other carotenoid producing species Cystofilobasidium capitatum , Sporobolomyces salmonicolor , and S. roseus were active only against about 40 % of the tested strains and exhibited weak activity .
	manualset3
157887	4	411341	7	NULL	NULL	0	NULL	S. roseus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The other carotenoid producing species Cystofilobasidium capitatum , Sporobolomyces salmonicolor , and S. roseus were active only against about 40 % of the tested strains and exhibited weak activity .
	manualset3
157889	6	411341	7	NULL	NULL	0	NULL	40 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The other carotenoid producing species Cystofilobasidium capitatum , Sporobolomyces salmonicolor , and S. roseus were active only against about 40 % of the tested strains and exhibited weak activity .
	manualset3
157890	7	411341	7	NULL	NULL	0	NULL	tested strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The other carotenoid producing species Cystofilobasidium capitatum , Sporobolomyces salmonicolor , and S. roseus were active only against about 40 % of the tested strains and exhibited weak activity .
	manualset3
157891	8	411341	7	NULL	NULL	0	NULL	weak activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The other carotenoid producing species Cystofilobasidium capitatum , Sporobolomyces salmonicolor , and S. roseus were active only against about 40 % of the tested strains and exhibited weak activity .
	manualset3
157892	1	411342	7	NULL	NULL	0	NULL	ACNU	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	ACNU and BCNU provoke the formation of DNA double-strand breaks ( DSB ) in glioma cells that precede the onset of apoptosis and necrosis .
	manualset3
157893	2	411342	7	NULL	NULL	0	NULL	BCNU	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	ACNU and BCNU provoke the formation of DNA double-strand breaks ( DSB ) in glioma cells that precede the onset of apoptosis and necrosis .
	manualset3
157894	3	411342	7	NULL	NULL	0	NULL	formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	ACNU and BCNU provoke the formation of DNA double-strand breaks ( DSB ) in glioma cells that precede the onset of apoptosis and necrosis .
	manualset3
157895	4	411342	7	NULL	NULL	0	NULL	DNA double-strand breaks ( DSB )	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	ACNU and BCNU provoke the formation of DNA double-strand breaks ( DSB ) in glioma cells that precede the onset of apoptosis and necrosis .
	manualset3
157896	5	411342	7	NULL	NULL	0	NULL	glioma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	ACNU and BCNU provoke the formation of DNA double-strand breaks ( DSB ) in glioma cells that precede the onset of apoptosis and necrosis .
	manualset3
157897	6	411342	7	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	ACNU and BCNU provoke the formation of DNA double-strand breaks ( DSB ) in glioma cells that precede the onset of apoptosis and necrosis .
	manualset3
157898	7	411342	7	NULL	NULL	0	NULL	necrosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	ACNU and BCNU provoke the formation of DNA double-strand breaks ( DSB ) in glioma cells that precede the onset of apoptosis and necrosis .
	manualset3
158514	8	411342	7	NULL	NULL	0	NULL	onset 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	ACNU and BCNU provoke the formation of DNA double-strand breaks ( DSB ) in glioma cells that precede the onset of apoptosis and necrosis .
	manualset3
157900	1	411343	7	NULL	NULL	NULL	NULL	costimulatory signals	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The other is provided by costimulatory signals .
	manualset3
157902	1	411344	7	NULL	NULL	NULL	NULL	US diagnostic criteria	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The other two US diagnostic criteria were much less accurate than VC .
	manualset3
157904	2	411344	7	NULL	NULL	NULL	NULL	VC	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The other two US diagnostic criteria were much less accurate than VC .
	manualset3
157905	1	411345	7	NULL	NULL	NULL	NULL	ACTH levels	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ACTH and cortisol levels in the plasma of patients who were treated with PSL ( PSL ( + ) group , n = 18 ) were lower than those in the plasma of patients who were treated without PSL ( PSL ( - ) group , n = 29 ; P & lt ; 0.05 and P & lt ; 0.01 , respectively ) .
	manualset3
157906	2	411345	7	NULL	NULL	NULL	NULL	cortisol levels	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ACTH and cortisol levels in the plasma of patients who were treated with PSL ( PSL ( + ) group , n = 18 ) were lower than those in the plasma of patients who were treated without PSL ( PSL ( - ) group , n = 29 ; P & lt ; 0.05 and P & lt ; 0.01 , respectively ) .
	manualset3
157907	3	411345	7	NULL	NULL	NULL	NULL	plasma	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ACTH and cortisol levels in the plasma of patients who were treated with PSL ( PSL ( + ) group , n = 18 ) were lower than those in the plasma of patients who were treated without PSL ( PSL ( - ) group , n = 29 ; P & lt ; 0.05 and P & lt ; 0.01 , respectively ) .
	manualset3
157908	4	411345	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	ACTH and cortisol levels in the plasma of patients who were treated with PSL ( PSL ( + ) group , n = 18 ) were lower than those in the plasma of patients who were treated without PSL ( PSL ( - ) group , n = 29 ; P & lt ; 0.05 and P & lt ; 0.01 , respectively ) .
	manualset3
157909	5	411345	7	NULL	NULL	0	NULL	PSL ( PSL ( + ) group , n = 18 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	ACTH and cortisol levels in the plasma of patients who were treated with PSL ( PSL ( + ) group , n = 18 ) were lower than those in the plasma of patients who were treated without PSL ( PSL ( - ) group , n = 29 ; P & lt ; 0.05 and P & lt ; 0.01 , respectively ) .
	manualset3
157910	6	411345	7	NULL	NULL	0	NULL	plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	ACTH and cortisol levels in the plasma of patients who were treated with PSL ( PSL ( + ) group , n = 18 ) were lower than those in the plasma of patients who were treated without PSL ( PSL ( - ) group , n = 29 ; P & lt ; 0.05 and P & lt ; 0.01 , respectively ) .
	manualset3
157911	7	411345	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	ACTH and cortisol levels in the plasma of patients who were treated with PSL ( PSL ( + ) group , n = 18 ) were lower than those in the plasma of patients who were treated without PSL ( PSL ( - ) group , n = 29 ; P & lt ; 0.05 and P & lt ; 0.01 , respectively ) .
	manualset3
157912	8	411345	7	NULL	NULL	0	NULL	PSL ( PSL ( - ) group , n = 29 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	ACTH and cortisol levels in the plasma of patients who were treated with PSL ( PSL ( + ) group , n = 18 ) were lower than those in the plasma of patients who were treated without PSL ( PSL ( - ) group , n = 29 ; P & lt ; 0.05 and P & lt ; 0.01 , respectively ) .
	manualset3
157913	9	411345	7	NULL	NULL	0	NULL	P & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	ACTH and cortisol levels in the plasma of patients who were treated with PSL ( PSL ( + ) group , n = 18 ) were lower than those in the plasma of patients who were treated without PSL ( PSL ( - ) group , n = 29 ; P & lt ; 0.05 and P & lt ; 0.01 , respectively ) .
	manualset3
157914	10	411345	7	NULL	NULL	0	NULL	P & lt ; 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	ACTH and cortisol levels in the plasma of patients who were treated with PSL ( PSL ( + ) group , n = 18 ) were lower than those in the plasma of patients who were treated without PSL ( PSL ( - ) group , n = 29 ; P & lt ; 0.05 and P & lt ; 0.01 , respectively ) .
	manualset3
157916	2	411346	7	NULL	NULL	0	NULL	two systems	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The other two systems are based on a receptor with selenium .
	manualset3
157917	3	411346	7	NULL	NULL	0	NULL	receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The other two systems are based on a receptor with selenium .
	manualset3
157918	4	411346	7	NULL	NULL	0	NULL	selenium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The other two systems are based on a receptor with selenium .
	manualset3
157919	1	411347	7	NULL	NULL	0	NULL	outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The outcome of a randomized clinical trial demonstrating that fetoscopic laser coagulation of chorionic plate vessels is the most effective treatment for twin-twin transfusion syndrome ( TTTS ) has revived interest in endoscopic fetal therapy .
	manualset3
157920	2	411347	7	NULL	NULL	NULL	NULL	 randomized clinical trial	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The outcome of a randomized clinical trial demonstrating that fetoscopic laser coagulation of chorionic plate vessels is the most effective treatment for twin-twin transfusion syndrome ( TTTS ) has revived interest in endoscopic fetal therapy .
	manualset3
157921	3	411347	7	NULL	NULL	NULL	NULL	fetoscopic laser coagulation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The outcome of a randomized clinical trial demonstrating that fetoscopic laser coagulation of chorionic plate vessels is the most effective treatment for twin-twin transfusion syndrome ( TTTS ) has revived interest in endoscopic fetal therapy .
	manualset3
157922	4	411347	7	NULL	NULL	0	NULL	chorionic plate vessels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The outcome of a randomized clinical trial demonstrating that fetoscopic laser coagulation of chorionic plate vessels is the most effective treatment for twin-twin transfusion syndrome ( TTTS ) has revived interest in endoscopic fetal therapy .
	manualset3
157923	5	411347	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The outcome of a randomized clinical trial demonstrating that fetoscopic laser coagulation of chorionic plate vessels is the most effective treatment for twin-twin transfusion syndrome ( TTTS ) has revived interest in endoscopic fetal therapy .
	manualset3
157924	6	411347	7	NULL	NULL	0	NULL	twin-twin transfusion syndrome ( TTTS )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The outcome of a randomized clinical trial demonstrating that fetoscopic laser coagulation of chorionic plate vessels is the most effective treatment for twin-twin transfusion syndrome ( TTTS ) has revived interest in endoscopic fetal therapy .
	manualset3
157925	7	411347	7	NULL	NULL	0	NULL	interest	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The outcome of a randomized clinical trial demonstrating that fetoscopic laser coagulation of chorionic plate vessels is the most effective treatment for twin-twin transfusion syndrome ( TTTS ) has revived interest in endoscopic fetal therapy .
	manualset3
157926	8	411347	7	NULL	NULL	0	NULL	endoscopic fetal therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The outcome of a randomized clinical trial demonstrating that fetoscopic laser coagulation of chorionic plate vessels is the most effective treatment for twin-twin transfusion syndrome ( TTTS ) has revived interest in endoscopic fetal therapy .
	manualset3
157927	1	411348	7	NULL	NULL	0	NULL	 outcome	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The outcome of diol oxidation reactions of some N-oxide diolchlorins varies from the corresponding reactions of the parent diolchlorins .
	manualset3
157928	2	411348	7	NULL	NULL	0	NULL	diol oxidation reactions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The outcome of diol oxidation reactions of some N-oxide diolchlorins varies from the corresponding reactions of the parent diolchlorins .
	manualset3
157929	3	411348	7	NULL	NULL	0	NULL	N-oxide diolchlorins	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The outcome of diol oxidation reactions of some N-oxide diolchlorins varies from the corresponding reactions of the parent diolchlorins .
	manualset3
157930	4	411348	7	NULL	NULL	0	NULL	reactions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The outcome of diol oxidation reactions of some N-oxide diolchlorins varies from the corresponding reactions of the parent diolchlorins .
	manualset3
157931	5	411348	7	NULL	NULL	0	NULL	parent diolchlorins	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The outcome of diol oxidation reactions of some N-oxide diolchlorins varies from the corresponding reactions of the parent diolchlorins .
	manualset3
157932	1	411349	7	NULL	NULL	0	NULL	outcome	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The outcome of the first pilot study of liver-directed gene therapy is reported here .
	manualset3
157933	2	411349	7	NULL	NULL	0	NULL	first pilot study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The outcome of the first pilot study of liver-directed gene therapy is reported here .
	manualset3
157934	3	411349	7	NULL	NULL	0	NULL	liver-directed gene therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The outcome of the first pilot study of liver-directed gene therapy is reported here .
	manualset3
157935	1	411350	7	NULL	NULL	0	NULL	 outcome	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The outcome of the study leads to the conclusion that PAS and OW are both suitable for quick screening of TAC in sour cherries .
	manualset3
157936	2	411350	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The outcome of the study leads to the conclusion that PAS and OW are both suitable for quick screening of TAC in sour cherries .
	manualset3
157937	3	411350	7	NULL	NULL	0	NULL	conclusion	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The outcome of the study leads to the conclusion that PAS and OW are both suitable for quick screening of TAC in sour cherries .
	manualset3
157938	4	411350	7	NULL	NULL	0	NULL	PAS	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The outcome of the study leads to the conclusion that PAS and OW are both suitable for quick screening of TAC in sour cherries .
	manualset3
157939	5	411350	7	NULL	NULL	0	NULL	OW	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The outcome of the study leads to the conclusion that PAS and OW are both suitable for quick screening of TAC in sour cherries .
	manualset3
157940	6	411350	7	NULL	NULL	0	NULL	TAC	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The outcome of the study leads to the conclusion that PAS and OW are both suitable for quick screening of TAC in sour cherries .
	manualset3
157941	7	411350	7	NULL	NULL	0	NULL	sour cherries	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The outcome of the study leads to the conclusion that PAS and OW are both suitable for quick screening of TAC in sour cherries .
	manualset3
157942	1	411351	7	NULL	NULL	0	NULL	outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The outcome was fatal in all cases with death resulting from refractory myocardial failure .
	manualset3
157943	2	411351	7	NULL	NULL	0	NULL	fatal	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The outcome was fatal in all cases with death resulting from refractory myocardial failure .
	manualset3
157944	3	411351	7	NULL	NULL	0	NULL	death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The outcome was fatal in all cases with death resulting from refractory myocardial failure .
	manualset3
157945	4	411351	7	NULL	NULL	0	NULL	refractory myocardial failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The outcome was fatal in all cases with death resulting from refractory myocardial failure .
	manualset3
157946	1	411352	7	NULL	NULL	0	NULL	outcomes 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The outcomes of ovarian cancer treatment are better when provided by gynecologic oncologists and in specialized hospitals : a systematic review .
	manualset3
157947	2	411352	7	NULL	NULL	0	NULL	ovarian cancer treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The outcomes of ovarian cancer treatment are better when provided by gynecologic oncologists and in specialized hospitals : a systematic review .
	manualset3
157948	3	411352	7	NULL	NULL	0	NULL	gynecologic oncologists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The outcomes of ovarian cancer treatment are better when provided by gynecologic oncologists and in specialized hospitals : a systematic review .
	manualset3
157949	4	411352	7	NULL	NULL	0	NULL	specialized hospitals	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The outcomes of ovarian cancer treatment are better when provided by gynecologic oncologists and in specialized hospitals : a systematic review .
	manualset3
157950	5	411352	7	NULL	NULL	NULL	NULL	systematic review	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The outcomes of ovarian cancer treatment are better when provided by gynecologic oncologists and in specialized hospitals : a systematic review .
	manualset3
157951	1	411353	7	NULL	NULL	0	NULL	output 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The output of the algorithm is a small number of template images that represent different modes in a population .
	manualset3
157952	2	411353	7	NULL	NULL	0	NULL	algorithm	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The output of the algorithm is a small number of template images that represent different modes in a population .
	manualset3
157953	3	411353	7	NULL	NULL	0	NULL	small number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The output of the algorithm is a small number of template images that represent different modes in a population .
	manualset3
157954	4	411353	7	NULL	NULL	0	NULL	template images	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The output of the algorithm is a small number of template images that represent different modes in a population .
	manualset3
157955	5	411353	7	NULL	NULL	0	NULL	population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The output of the algorithm is a small number of template images that represent different modes in a population .
	manualset3
157956	1	411354	7	NULL	NULL	0	NULL	outward current 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The outward current is partially blocked by 1 mM 4-aminopyridine but not TEA or curare .
	manualset3
157957	2	411354	7	NULL	NULL	0	NULL	 1 mM 4-aminopyridine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The outward current is partially blocked by 1 mM 4-aminopyridine but not TEA or curare .
	manualset3
157958	3	411354	7	NULL	NULL	0	NULL	TEA 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The outward current is partially blocked by 1 mM 4-aminopyridine but not TEA or curare .
	manualset3
157959	4	411354	7	NULL	NULL	0	NULL	curare	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The outward current is partially blocked by 1 mM 4-aminopyridine but not TEA or curare .
	manualset3
157960	1	411355	7	NULL	NULL	0	NULL	 outward pathways of glycine	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The outward pathways of glycine from the total body free glycine pool are conversion to other amino acids and oxidation to excretory end products ( 30 % to 42 % ) and incorporation into protein , which accounts for 45 % to 61 % of glycine N loss from the metabolic pool .
	manualset3
157961	2	411355	7	NULL	NULL	0	NULL	total body free glycine pool	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The outward pathways of glycine from the total body free glycine pool are conversion to other amino acids and oxidation to excretory end products ( 30 % to 42 % ) and incorporation into protein , which accounts for 45 % to 61 % of glycine N loss from the metabolic pool .
	manualset3
157962	3	411355	7	NULL	NULL	0	NULL	amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The outward pathways of glycine from the total body free glycine pool are conversion to other amino acids and oxidation to excretory end products ( 30 % to 42 % ) and incorporation into protein , which accounts for 45 % to 61 % of glycine N loss from the metabolic pool .
	manualset3
157963	4	411355	7	NULL	NULL	0	NULL	oxidation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The outward pathways of glycine from the total body free glycine pool are conversion to other amino acids and oxidation to excretory end products ( 30 % to 42 % ) and incorporation into protein , which accounts for 45 % to 61 % of glycine N loss from the metabolic pool .
	manualset3
157964	5	411355	7	NULL	NULL	0	NULL	excretory end products	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The outward pathways of glycine from the total body free glycine pool are conversion to other amino acids and oxidation to excretory end products ( 30 % to 42 % ) and incorporation into protein , which accounts for 45 % to 61 % of glycine N loss from the metabolic pool .
	manualset3
157965	6	411355	7	NULL	NULL	NULL	NULL	30 % to 42 % 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The outward pathways of glycine from the total body free glycine pool are conversion to other amino acids and oxidation to excretory end products ( 30 % to 42 % ) and incorporation into protein , which accounts for 45 % to 61 % of glycine N loss from the metabolic pool .
	manualset3
157966	7	411355	7	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The outward pathways of glycine from the total body free glycine pool are conversion to other amino acids and oxidation to excretory end products ( 30 % to 42 % ) and incorporation into protein , which accounts for 45 % to 61 % of glycine N loss from the metabolic pool .
	manualset3
157967	8	411355	7	NULL	NULL	NULL	NULL	45 % to 61 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The outward pathways of glycine from the total body free glycine pool are conversion to other amino acids and oxidation to excretory end products ( 30 % to 42 % ) and incorporation into protein , which accounts for 45 % to 61 % of glycine N loss from the metabolic pool .
	manualset3
157968	9	411355	7	NULL	NULL	0	NULL	glycine N loss	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The outward pathways of glycine from the total body free glycine pool are conversion to other amino acids and oxidation to excretory end products ( 30 % to 42 % ) and incorporation into protein , which accounts for 45 % to 61 % of glycine N loss from the metabolic pool .
	manualset3
157969	10	411355	7	NULL	NULL	NULL	NULL	metabolic pool 	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The outward pathways of glycine from the total body free glycine pool are conversion to other amino acids and oxidation to excretory end products ( 30 % to 42 % ) and incorporation into protein , which accounts for 45 % to 61 % of glycine N loss from the metabolic pool .
	manualset3
161003	11	411355	7	NULL	NULL	0	NULL	conversion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The outward pathways of glycine from the total body free glycine pool are conversion to other amino acids and oxidation to excretory end products ( 30 % to 42 % ) and incorporation into protein , which accounts for 45 % to 61 % of glycine N loss from the metabolic pool .
	manualset3
161004	12	411355	7	NULL	NULL	0	NULL	incorporation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The outward pathways of glycine from the total body free glycine pool are conversion to other amino acids and oxidation to excretory end products ( 30 % to 42 % ) and incorporation into protein , which accounts for 45 % to 61 % of glycine N loss from the metabolic pool .
	manualset3
157970	1	411356	7	NULL	NULL	0	NULL	ovaries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The ovaries were recovered at 14 days after the second PG ( luteal phase ) or 24h after the third PG given 14 days after the second PG ( follicular phase ) .
	manualset3
157971	2	411356	7	NULL	NULL	0	NULL	14 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The ovaries were recovered at 14 days after the second PG ( luteal phase ) or 24h after the third PG given 14 days after the second PG ( follicular phase ) .
	manualset3
157972	3	411356	7	NULL	NULL	NULL	NULL	second PG ( luteal phase ) 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ovaries were recovered at 14 days after the second PG ( luteal phase ) or 24h after the third PG given 14 days after the second PG ( follicular phase ) .
	manualset3
157973	4	411356	7	NULL	NULL	0	NULL	24h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The ovaries were recovered at 14 days after the second PG ( luteal phase ) or 24h after the third PG given 14 days after the second PG ( follicular phase ) .
	manualset3
157974	5	411356	7	NULL	NULL	0	NULL	third PG	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ovaries were recovered at 14 days after the second PG ( luteal phase ) or 24h after the third PG given 14 days after the second PG ( follicular phase ) .
	manualset3
157975	6	411356	7	NULL	NULL	0	NULL	14 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The ovaries were recovered at 14 days after the second PG ( luteal phase ) or 24h after the third PG given 14 days after the second PG ( follicular phase ) .
	manualset3
157976	7	411356	7	NULL	NULL	0	NULL	second PG ( follicular phase )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ovaries were recovered at 14 days after the second PG ( luteal phase ) or 24h after the third PG given 14 days after the second PG ( follicular phase ) .
	manualset3
157977	1	411357	7	NULL	NULL	0	NULL	chemosensitivity rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall chemosensitivity rate of LY 186641 was 37 % and the average tumor growth inhibition rates ( TGIRs ) of malignant lymphoma , esophageal cancer and colorectal cancer were 51 + / - 19 % , 51 + / - 20 % and 48 + / - 12 % , respectively .
	manualset3
157978	2	411357	7	NULL	NULL	0	NULL	LY 186641	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall chemosensitivity rate of LY 186641 was 37 % and the average tumor growth inhibition rates ( TGIRs ) of malignant lymphoma , esophageal cancer and colorectal cancer were 51 + / - 19 % , 51 + / - 20 % and 48 + / - 12 % , respectively .
	manualset3
157979	3	411357	7	NULL	NULL	0	NULL	37 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall chemosensitivity rate of LY 186641 was 37 % and the average tumor growth inhibition rates ( TGIRs ) of malignant lymphoma , esophageal cancer and colorectal cancer were 51 + / - 19 % , 51 + / - 20 % and 48 + / - 12 % , respectively .
	manualset3
157980	4	411357	7	NULL	NULL	0	NULL	 average tumor growth inhibition rates ( TGIRs ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall chemosensitivity rate of LY 186641 was 37 % and the average tumor growth inhibition rates ( TGIRs ) of malignant lymphoma , esophageal cancer and colorectal cancer were 51 + / - 19 % , 51 + / - 20 % and 48 + / - 12 % , respectively .
	manualset3
157981	5	411357	7	NULL	NULL	0	NULL	malignant lymphoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall chemosensitivity rate of LY 186641 was 37 % and the average tumor growth inhibition rates ( TGIRs ) of malignant lymphoma , esophageal cancer and colorectal cancer were 51 + / - 19 % , 51 + / - 20 % and 48 + / - 12 % , respectively .
	manualset3
157982	6	411357	7	NULL	NULL	0	NULL	esophageal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall chemosensitivity rate of LY 186641 was 37 % and the average tumor growth inhibition rates ( TGIRs ) of malignant lymphoma , esophageal cancer and colorectal cancer were 51 + / - 19 % , 51 + / - 20 % and 48 + / - 12 % , respectively .
	manualset3
157983	7	411357	7	NULL	NULL	0	NULL	colorectal cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall chemosensitivity rate of LY 186641 was 37 % and the average tumor growth inhibition rates ( TGIRs ) of malignant lymphoma , esophageal cancer and colorectal cancer were 51 + / - 19 % , 51 + / - 20 % and 48 + / - 12 % , respectively .
	manualset3
157984	8	411357	7	NULL	NULL	0	NULL	51 + / - 19 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall chemosensitivity rate of LY 186641 was 37 % and the average tumor growth inhibition rates ( TGIRs ) of malignant lymphoma , esophageal cancer and colorectal cancer were 51 + / - 19 % , 51 + / - 20 % and 48 + / - 12 % , respectively .
	manualset3
157985	9	411357	7	NULL	NULL	0	NULL	51 + / - 20 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall chemosensitivity rate of LY 186641 was 37 % and the average tumor growth inhibition rates ( TGIRs ) of malignant lymphoma , esophageal cancer and colorectal cancer were 51 + / - 19 % , 51 + / - 20 % and 48 + / - 12 % , respectively .
	manualset3
157986	10	411357	7	NULL	NULL	0	NULL	48 + / - 12 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall chemosensitivity rate of LY 186641 was 37 % and the average tumor growth inhibition rates ( TGIRs ) of malignant lymphoma , esophageal cancer and colorectal cancer were 51 + / - 19 % , 51 + / - 20 % and 48 + / - 12 % , respectively .
	manualset3
157987	1	411358	7	NULL	NULL	NULL	NULL	gene organization	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The overall gene organization was the same as the bovine and rabbit CYB5 genes .
	manualset3
157988	2	411358	7	NULL	NULL	0	NULL	bovine CYB5 genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall gene organization was the same as the bovine and rabbit CYB5 genes .
	manualset3
157989	3	411358	7	NULL	NULL	0	NULL	rabbit CYB5 genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall gene organization was the same as the bovine and rabbit CYB5 genes .
	manualset3
157990	1	411359	7	NULL	NULL	0	NULL	ACTH effects 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	ACTH effects were mimicked by nonspecific phospholipase C ( PLC ) .
	manualset3
157991	2	411359	7	NULL	NULL	0	NULL	nonspecific phospholipase C ( PLC )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	ACTH effects were mimicked by nonspecific phospholipase C ( PLC ) .
	manualset3
157992	1	411360	7	NULL	NULL	0	NULL	overall growth rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall growth rate of the cultures is influenced by a wide range of growth stimulatory and inhibitory molecules , but it is not clear whether responsiveness to these factors differs between the different subpopulations of dividing cells .
	manualset3
157994	2	411360	7	NULL	NULL	0	NULL	cultures	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall growth rate of the cultures is influenced by a wide range of growth stimulatory and inhibitory molecules , but it is not clear whether responsiveness to these factors differs between the different subpopulations of dividing cells .
	manualset3
157995	3	411360	7	NULL	NULL	0	NULL	growth stimulatory molecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall growth rate of the cultures is influenced by a wide range of growth stimulatory and inhibitory molecules , but it is not clear whether responsiveness to these factors differs between the different subpopulations of dividing cells .
	manualset3
157996	4	411360	7	NULL	NULL	NULL	NULL	growth inhibitory molecules	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The overall growth rate of the cultures is influenced by a wide range of growth stimulatory and inhibitory molecules , but it is not clear whether responsiveness to these factors differs between the different subpopulations of dividing cells .
	manualset3
157997	5	411360	7	NULL	NULL	NULL	NULL	subpopulations of dividing cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The overall growth rate of the cultures is influenced by a wide range of growth stimulatory and inhibitory molecules , but it is not clear whether responsiveness to these factors differs between the different subpopulations of dividing cells .
	manualset3
158515	6	411360	7	NULL	NULL	NULL	NULL	responsiveness 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The overall growth rate of the cultures is influenced by a wide range of growth stimulatory and inhibitory molecules , but it is not clear whether responsiveness to these factors differs between the different subpopulations of dividing cells .
	manualset3
158516	7	411360	7	NULL	NULL	NULL	NULL	factors	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The overall growth rate of the cultures is influenced by a wide range of growth stimulatory and inhibitory molecules , but it is not clear whether responsiveness to these factors differs between the different subpopulations of dividing cells .
	manualset3
157999	1	411361	7	NULL	NULL	0	NULL	prevalence data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall prevalence data were : 13.9 % for HIV ( 37 of 267 ) , 22.8 % for syphilis ( 66 of 290 ) , and 16.2 % for HCV ( 47 of 290 ) .
	manualset3
158000	2	411361	7	NULL	NULL	0	NULL	13.9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall prevalence data were : 13.9 % for HIV ( 37 of 267 ) , 22.8 % for syphilis ( 66 of 290 ) , and 16.2 % for HCV ( 47 of 290 ) .
	manualset3
158001	3	411361	7	NULL	NULL	0	NULL	HIV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall prevalence data were : 13.9 % for HIV ( 37 of 267 ) , 22.8 % for syphilis ( 66 of 290 ) , and 16.2 % for HCV ( 47 of 290 ) .
	manualset3
158002	4	411361	7	NULL	NULL	0	NULL	37 of 267	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall prevalence data were : 13.9 % for HIV ( 37 of 267 ) , 22.8 % for syphilis ( 66 of 290 ) , and 16.2 % for HCV ( 47 of 290 ) .
	manualset3
158003	5	411361	7	NULL	NULL	0	NULL	 22.8 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall prevalence data were : 13.9 % for HIV ( 37 of 267 ) , 22.8 % for syphilis ( 66 of 290 ) , and 16.2 % for HCV ( 47 of 290 ) .
	manualset3
158004	6	411361	7	NULL	NULL	0	NULL	syphilis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall prevalence data were : 13.9 % for HIV ( 37 of 267 ) , 22.8 % for syphilis ( 66 of 290 ) , and 16.2 % for HCV ( 47 of 290 ) .
	manualset3
158005	7	411361	7	NULL	NULL	0	NULL	66 of 290	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall prevalence data were : 13.9 % for HIV ( 37 of 267 ) , 22.8 % for syphilis ( 66 of 290 ) , and 16.2 % for HCV ( 47 of 290 ) .
	manualset3
158006	8	411361	7	NULL	NULL	0	NULL	16.2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall prevalence data were : 13.9 % for HIV ( 37 of 267 ) , 22.8 % for syphilis ( 66 of 290 ) , and 16.2 % for HCV ( 47 of 290 ) .
	manualset3
158007	9	411361	7	NULL	NULL	0	NULL	HCV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall prevalence data were : 13.9 % for HIV ( 37 of 267 ) , 22.8 % for syphilis ( 66 of 290 ) , and 16.2 % for HCV ( 47 of 290 ) .
	manualset3
158008	10	411361	7	NULL	NULL	0	NULL	47 of 290	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall prevalence data were : 13.9 % for HIV ( 37 of 267 ) , 22.8 % for syphilis ( 66 of 290 ) , and 16.2 % for HCV ( 47 of 290 ) .
	manualset3
158009	1	411362	7	NULL	NULL	0	NULL	MRSA infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall prevalence of MRSA infection was 34 % .
	manualset3
158010	2	411362	7	NULL	NULL	0	NULL	34 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall prevalence of MRSA infection was 34 % .
	manualset3
161005	3	411362	7	NULL	NULL	0	NULL	prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall prevalence of MRSA infection was 34 % .
	manualset3
158011	1	411363	7	NULL	NULL	NULL	NULL	results	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The overall results showed that the GSTM1 null was related to an increased risk of cervical cancer ( OR = 1.50 , 95 % CI = 1.21-1 .85 ) .
	manualset3
158012	2	411363	7	NULL	NULL	0	NULL	GSTM1 null 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall results showed that the GSTM1 null was related to an increased risk of cervical cancer ( OR = 1.50 , 95 % CI = 1.21-1 .85 ) .
	manualset3
158013	3	411363	7	NULL	NULL	0	NULL	cervical cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall results showed that the GSTM1 null was related to an increased risk of cervical cancer ( OR = 1.50 , 95 % CI = 1.21-1 .85 ) .
	manualset3
158014	4	411363	7	NULL	NULL	NULL	NULL	OR = 1.50 , 95 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The overall results showed that the GSTM1 null was related to an increased risk of cervical cancer ( OR = 1.50 , 95 % CI = 1.21-1 .85 ) .
	manualset3
158015	5	411363	7	NULL	NULL	0	NULL	 CI = 1.21-1 .85 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall results showed that the GSTM1 null was related to an increased risk of cervical cancer ( OR = 1.50 , 95 % CI = 1.21-1 .85 ) .
	manualset3
158517	6	411363	7	NULL	NULL	0	NULL	increased risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The overall results showed that the GSTM1 null was related to an increased risk of cervical cancer ( OR = 1.50 , 95 % CI = 1.21-1 .85 ) .
	manualset3
158016	1	411364	7	NULL	NULL	0	NULL	overexpressed IRS-I protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The overexpressed IRS-I protein was highly tyrosyl phosphorylated following insulin/insulin - like growth factor I stimulation and led to constitutive activation of downstream signal transduction molecules such as phosphatidylinositol-3 kinase and mitogen-activated protein kinase .
	manualset3
158017	2	411364	7	NULL	NULL	NULL	NULL	insulin/insulin - like growth factor I stimulation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The overexpressed IRS-I protein was highly tyrosyl phosphorylated following insulin/insulin - like growth factor I stimulation and led to constitutive activation of downstream signal transduction molecules such as phosphatidylinositol-3 kinase and mitogen-activated protein kinase .
	manualset3
158018	3	411364	7	NULL	NULL	NULL	NULL	downstream signal transduction molecules	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The overexpressed IRS-I protein was highly tyrosyl phosphorylated following insulin/insulin - like growth factor I stimulation and led to constitutive activation of downstream signal transduction molecules such as phosphatidylinositol-3 kinase and mitogen-activated protein kinase .
	manualset3
158019	4	411364	7	NULL	NULL	0	NULL	phosphatidylinositol-3 kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The overexpressed IRS-I protein was highly tyrosyl phosphorylated following insulin/insulin - like growth factor I stimulation and led to constitutive activation of downstream signal transduction molecules such as phosphatidylinositol-3 kinase and mitogen-activated protein kinase .
	manualset3
158020	5	411364	7	NULL	NULL	0	NULL	mitogen-activated protein kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The overexpressed IRS-I protein was highly tyrosyl phosphorylated following insulin/insulin - like growth factor I stimulation and led to constitutive activation of downstream signal transduction molecules such as phosphatidylinositol-3 kinase and mitogen-activated protein kinase .
	manualset3
158518	6	411364	7	NULL	NULL	0	NULL	highly tyrosyl phosphorylated	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The overexpressed IRS-I protein was highly tyrosyl phosphorylated following insulin/insulin - like growth factor I stimulation and led to constitutive activation of downstream signal transduction molecules such as phosphatidylinositol-3 kinase and mitogen-activated protein kinase .
	manualset3
158519	7	411364	7	NULL	NULL	0	NULL	constitutive activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The overexpressed IRS-I protein was highly tyrosyl phosphorylated following insulin/insulin - like growth factor I stimulation and led to constitutive activation of downstream signal transduction molecules such as phosphatidylinositol-3 kinase and mitogen-activated protein kinase .
	manualset3
158021	1	411365	7	NULL	NULL	0	NULL	oxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The oxidation of anti-inflammatory drugs such Indomethacin and Ibuprofen was carried out successfully and the decarboxylated products were obtained .
	manualset3
158022	2	411365	7	NULL	NULL	0	NULL	anti-inflammatory drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The oxidation of anti-inflammatory drugs such Indomethacin and Ibuprofen was carried out successfully and the decarboxylated products were obtained .
	manualset3
158023	3	411365	7	NULL	NULL	0	NULL	Indomethacin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The oxidation of anti-inflammatory drugs such Indomethacin and Ibuprofen was carried out successfully and the decarboxylated products were obtained .
	manualset3
158024	4	411365	7	NULL	NULL	0	NULL	Ibuprofen	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The oxidation of anti-inflammatory drugs such Indomethacin and Ibuprofen was carried out successfully and the decarboxylated products were obtained .
	manualset3
158025	5	411365	7	NULL	NULL	0	NULL	decarboxylated products	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The oxidation of anti-inflammatory drugs such Indomethacin and Ibuprofen was carried out successfully and the decarboxylated products were obtained .
	manualset3
158026	1	411366	7	NULL	NULL	0	NULL	oxygen atoms	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The oxygen atoms in oligoEGs were found to act as Lewis bases on the metal cations to produce the `` flexible '' nucleophile , whereas the two terminal hydroxy ( OH ) groups acted as `` anchors '' to orientate the nucleophile and the substrate into an ideal configuration for the reaction .
	manualset3
158027	2	411366	7	NULL	NULL	0	NULL	oligoEGs	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The oxygen atoms in oligoEGs were found to act as Lewis bases on the metal cations to produce the `` flexible '' nucleophile , whereas the two terminal hydroxy ( OH ) groups acted as `` anchors '' to orientate the nucleophile and the substrate into an ideal configuration for the reaction .
	manualset3
158028	3	411366	7	NULL	NULL	0	NULL	Lewis bases	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The oxygen atoms in oligoEGs were found to act as Lewis bases on the metal cations to produce the `` flexible '' nucleophile , whereas the two terminal hydroxy ( OH ) groups acted as `` anchors '' to orientate the nucleophile and the substrate into an ideal configuration for the reaction .
	manualset3
158029	4	411366	7	NULL	NULL	0	NULL	metal cations	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The oxygen atoms in oligoEGs were found to act as Lewis bases on the metal cations to produce the `` flexible '' nucleophile , whereas the two terminal hydroxy ( OH ) groups acted as `` anchors '' to orientate the nucleophile and the substrate into an ideal configuration for the reaction .
	manualset3
158030	5	411366	7	NULL	NULL	NULL	NULL	 `` flexible '' nucleophile	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The oxygen atoms in oligoEGs were found to act as Lewis bases on the metal cations to produce the `` flexible '' nucleophile , whereas the two terminal hydroxy ( OH ) groups acted as `` anchors '' to orientate the nucleophile and the substrate into an ideal configuration for the reaction .
	manualset3
158031	6	411366	7	NULL	NULL	0	NULL	two terminal hydroxy ( OH ) groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The oxygen atoms in oligoEGs were found to act as Lewis bases on the metal cations to produce the `` flexible '' nucleophile , whereas the two terminal hydroxy ( OH ) groups acted as `` anchors '' to orientate the nucleophile and the substrate into an ideal configuration for the reaction .
	manualset3
158032	7	411366	7	NULL	NULL	NULL	NULL	anchors	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The oxygen atoms in oligoEGs were found to act as Lewis bases on the metal cations to produce the `` flexible '' nucleophile , whereas the two terminal hydroxy ( OH ) groups acted as `` anchors '' to orientate the nucleophile and the substrate into an ideal configuration for the reaction .
	manualset3
158033	8	411366	7	NULL	NULL	0	NULL	nucleophile	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The oxygen atoms in oligoEGs were found to act as Lewis bases on the metal cations to produce the `` flexible '' nucleophile , whereas the two terminal hydroxy ( OH ) groups acted as `` anchors '' to orientate the nucleophile and the substrate into an ideal configuration for the reaction .
	manualset3
158034	9	411366	7	NULL	NULL	NULL	NULL	substrate 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The oxygen atoms in oligoEGs were found to act as Lewis bases on the metal cations to produce the `` flexible '' nucleophile , whereas the two terminal hydroxy ( OH ) groups acted as `` anchors '' to orientate the nucleophile and the substrate into an ideal configuration for the reaction .
	manualset3
158035	10	411366	7	NULL	NULL	0	NULL	ideal configuration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The oxygen atoms in oligoEGs were found to act as Lewis bases on the metal cations to produce the `` flexible '' nucleophile , whereas the two terminal hydroxy ( OH ) groups acted as `` anchors '' to orientate the nucleophile and the substrate into an ideal configuration for the reaction .
	manualset3
158036	11	411366	7	NULL	NULL	0	NULL	 reaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The oxygen atoms in oligoEGs were found to act as Lewis bases on the metal cations to produce the `` flexible '' nucleophile , whereas the two terminal hydroxy ( OH ) groups acted as `` anchors '' to orientate the nucleophile and the substrate into an ideal configuration for the reaction .
	manualset3
158037	1	411367	7	NULL	NULL	0	NULL	ACh activated Ca2 + - regulated exocytosis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	ACh activated Ca2 + - regulated exocytosis ( an initial phase followed by a sustained phase ) .
	manualset3
158038	2	411367	7	NULL	NULL	NULL	NULL	 initial phase 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ACh activated Ca2 + - regulated exocytosis ( an initial phase followed by a sustained phase ) .
	manualset3
161006	3	411367	7	NULL	NULL	0	NULL	sustained phase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	ACh activated Ca2 + - regulated exocytosis ( an initial phase followed by a sustained phase ) .
	manualset3
158039	1	411368	7	NULL	NULL	0	NULL	p300/CBP cofactors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The p300/CBP cofactors are involved in a plethora of physiological processes , and their activity is essential for embryogenesis .
	manualset3
158040	2	411368	7	NULL	NULL	0	NULL	 physiological processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The p300/CBP cofactors are involved in a plethora of physiological processes , and their activity is essential for embryogenesis .
	manualset3
158041	3	411368	7	NULL	NULL	0	NULL	activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The p300/CBP cofactors are involved in a plethora of physiological processes , and their activity is essential for embryogenesis .
	manualset3
158042	4	411368	7	NULL	NULL	0	NULL	embryogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The p300/CBP cofactors are involved in a plethora of physiological processes , and their activity is essential for embryogenesis .
	manualset3
158043	1	411369	7	NULL	NULL	0	NULL	 pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The pH of the vancomycin solution changed too quickly for storage to be recommended .
	manualset3
158044	2	411369	7	NULL	NULL	0	NULL	vancomycin solution	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The pH of the vancomycin solution changed too quickly for storage to be recommended .
	manualset3
158045	3	411369	7	NULL	NULL	0	NULL	 storage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The pH of the vancomycin solution changed too quickly for storage to be recommended .
	manualset3
158046	1	411370	7	NULL	NULL	0	NULL	pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The pH was recorded for 1 hr in the fasted state , a standard liquid and solid meal of 1000 cal was given over 30 min , then the pH was measured for 4 hr postprandially .
	manualset3
158047	2	411370	7	NULL	NULL	0	NULL	1 hr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The pH was recorded for 1 hr in the fasted state , a standard liquid and solid meal of 1000 cal was given over 30 min , then the pH was measured for 4 hr postprandially .
	manualset3
158048	3	411370	7	NULL	NULL	0	NULL	fasted state	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The pH was recorded for 1 hr in the fasted state , a standard liquid and solid meal of 1000 cal was given over 30 min , then the pH was measured for 4 hr postprandially .
	manualset3
158049	4	411370	7	NULL	NULL	0	NULL	standard liquid	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The pH was recorded for 1 hr in the fasted state , a standard liquid and solid meal of 1000 cal was given over 30 min , then the pH was measured for 4 hr postprandially .
	manualset3
158050	5	411370	7	NULL	NULL	0	NULL	standard solid meal	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The pH was recorded for 1 hr in the fasted state , a standard liquid and solid meal of 1000 cal was given over 30 min , then the pH was measured for 4 hr postprandially .
	manualset3
158051	6	411370	7	NULL	NULL	0	NULL	1000 cal	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The pH was recorded for 1 hr in the fasted state , a standard liquid and solid meal of 1000 cal was given over 30 min , then the pH was measured for 4 hr postprandially .
	manualset3
158052	7	411370	7	NULL	NULL	0	NULL	30 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The pH was recorded for 1 hr in the fasted state , a standard liquid and solid meal of 1000 cal was given over 30 min , then the pH was measured for 4 hr postprandially .
	manualset3
158053	8	411370	7	NULL	NULL	0	NULL	pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The pH was recorded for 1 hr in the fasted state , a standard liquid and solid meal of 1000 cal was given over 30 min , then the pH was measured for 4 hr postprandially .
	manualset3
158054	9	411370	7	NULL	NULL	0	NULL	4 hr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The pH was recorded for 1 hr in the fasted state , a standard liquid and solid meal of 1000 cal was given over 30 min , then the pH was measured for 4 hr postprandially .
	manualset3
158055	1	411371	7	NULL	NULL	0	NULL	pKa	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The pKa of batrachotoxinin-A , an analog of BTX-B , was found by titrimetric methods to be greater than or equal to 8.2 .
	manualset3
158056	2	411371	7	NULL	NULL	0	NULL	 batrachotoxinin-A 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The pKa of batrachotoxinin-A , an analog of BTX-B , was found by titrimetric methods to be greater than or equal to 8.2 .
	manualset3
158057	3	411371	7	NULL	NULL	0	NULL	analog of BTX-B	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The pKa of batrachotoxinin-A , an analog of BTX-B , was found by titrimetric methods to be greater than or equal to 8.2 .
	manualset3
158058	4	411371	7	NULL	NULL	0	NULL	titrimetric methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The pKa of batrachotoxinin-A , an analog of BTX-B , was found by titrimetric methods to be greater than or equal to 8.2 .
	manualset3
158059	5	411371	7	NULL	NULL	0	NULL	8.2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The pKa of batrachotoxinin-A , an analog of BTX-B , was found by titrimetric methods to be greater than or equal to 8.2 .
	manualset3
158060	1	411372	7	NULL	NULL	0	NULL	 pKa1 values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The pKa1 values in the pH-activity profiles of the wild-type and mutant enzymes were 6.41 , 6.54 , and 6.65 for wild-type , Y121F , and Y121H , respectively .
	manualset3
158061	2	411372	7	NULL	NULL	0	NULL	pH-activity profiles	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The pKa1 values in the pH-activity profiles of the wild-type and mutant enzymes were 6.41 , 6.54 , and 6.65 for wild-type , Y121F , and Y121H , respectively .
	manualset3
158062	3	411372	7	NULL	NULL	0	NULL	 wild-type enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The pKa1 values in the pH-activity profiles of the wild-type and mutant enzymes were 6.41 , 6.54 , and 6.65 for wild-type , Y121F , and Y121H , respectively .
	manualset3
158063	4	411372	7	NULL	NULL	0	NULL	mutant enzymes	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The pKa1 values in the pH-activity profiles of the wild-type and mutant enzymes were 6.41 , 6.54 , and 6.65 for wild-type , Y121F , and Y121H , respectively .
	manualset3
158064	5	411372	7	NULL	NULL	0	NULL	6.41	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The pKa1 values in the pH-activity profiles of the wild-type and mutant enzymes were 6.41 , 6.54 , and 6.65 for wild-type , Y121F , and Y121H , respectively .
	manualset3
158065	6	411372	7	NULL	NULL	0	NULL	 6.54	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The pKa1 values in the pH-activity profiles of the wild-type and mutant enzymes were 6.41 , 6.54 , and 6.65 for wild-type , Y121F , and Y121H , respectively .
	manualset3
158066	7	411372	7	NULL	NULL	0	NULL	6.65 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The pKa1 values in the pH-activity profiles of the wild-type and mutant enzymes were 6.41 , 6.54 , and 6.65 for wild-type , Y121F , and Y121H , respectively .
	manualset3
158067	8	411372	7	NULL	NULL	NULL	NULL	wild-type	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The pKa1 values in the pH-activity profiles of the wild-type and mutant enzymes were 6.41 , 6.54 , and 6.65 for wild-type , Y121F , and Y121H , respectively .
	manualset3
158068	9	411372	7	NULL	NULL	0	NULL	 Y121F	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The pKa1 values in the pH-activity profiles of the wild-type and mutant enzymes were 6.41 , 6.54 , and 6.65 for wild-type , Y121F , and Y121H , respectively .
	manualset3
158069	10	411372	7	NULL	NULL	0	NULL	 Y121H	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The pKa1 values in the pH-activity profiles of the wild-type and mutant enzymes were 6.41 , 6.54 , and 6.65 for wild-type , Y121F , and Y121H , respectively .
	manualset3
158070	1	411373	7	NULL	NULL	0	NULL	 pMMO-activity assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The pMMO-activity assays indicated that the ( Cu , Zn ) - pMMO was no longer capable of supporting catalytic turnover of hydrocarbon substrates .
	manualset3
158071	2	411373	7	NULL	NULL	0	NULL	 ( Cu , Zn ) - pMMO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The pMMO-activity assays indicated that the ( Cu , Zn ) - pMMO was no longer capable of supporting catalytic turnover of hydrocarbon substrates .
	manualset3
158072	3	411373	7	NULL	NULL	0	NULL	catalytic turnover	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The pMMO-activity assays indicated that the ( Cu , Zn ) - pMMO was no longer capable of supporting catalytic turnover of hydrocarbon substrates .
	manualset3
158073	4	411373	7	NULL	NULL	0	NULL	hydrocarbon substrates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The pMMO-activity assays indicated that the ( Cu , Zn ) - pMMO was no longer capable of supporting catalytic turnover of hydrocarbon substrates .
	manualset3
158074	1	411374	7	NULL	NULL	0	NULL	packaging signal 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The packaging signal of MLV is an integrated module that mediates intracellular transport of genomic RNAs .
	manualset3
158075	2	411374	7	NULL	NULL	0	NULL	MLV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The packaging signal of MLV is an integrated module that mediates intracellular transport of genomic RNAs .
	manualset3
158076	3	411374	7	NULL	NULL	0	NULL	intracellular transport	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The packaging signal of MLV is an integrated module that mediates intracellular transport of genomic RNAs .
	manualset3
158077	4	411374	7	NULL	NULL	0	NULL	genomic RNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The packaging signal of MLV is an integrated module that mediates intracellular transport of genomic RNAs .
	manualset3
158078	5	411374	7	NULL	NULL	NULL	NULL	integrated module	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The packaging signal of MLV is an integrated module that mediates intracellular transport of genomic RNAs .
	manualset3
158079	1	411375	7	NULL	NULL	0	NULL	pain response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The pain response was , therefore , examined in a rat model of obesity induced by palatable food high in unsaturated fats .
	manualset3
158080	2	411375	7	NULL	NULL	0	NULL	rat model of obesity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The pain response was , therefore , examined in a rat model of obesity induced by palatable food high in unsaturated fats .
	manualset3
158081	3	411375	7	NULL	NULL	0	NULL	palatable food 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The pain response was , therefore , examined in a rat model of obesity induced by palatable food high in unsaturated fats .
	manualset3
158082	4	411375	7	NULL	NULL	0	NULL	unsaturated fats	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The pain response was , therefore , examined in a rat model of obesity induced by palatable food high in unsaturated fats .
	manualset3
158083	1	411376	7	NULL	NULL	0	NULL	pairs of enantiomers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The pairs of enantiomers in the true kryptoracemates usually have very similar conformations ; often the match is near-perfect .
	manualset3
158084	2	411376	7	NULL	NULL	0	NULL	true kryptoracemates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The pairs of enantiomers in the true kryptoracemates usually have very similar conformations ; often the match is near-perfect .
	manualset3
158085	3	411376	7	NULL	NULL	0	NULL	similar conformations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The pairs of enantiomers in the true kryptoracemates usually have very similar conformations ; often the match is near-perfect .
	manualset3
158086	4	411376	7	NULL	NULL	NULL	NULL	match	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The pairs of enantiomers in the true kryptoracemates usually have very similar conformations ; often the match is near-perfect .
	manualset3
158087	5	411376	7	NULL	NULL	0	NULL	 near-perfect	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The pairs of enantiomers in the true kryptoracemates usually have very similar conformations ; often the match is near-perfect .
	manualset3
158088	1	411377	7	NULL	NULL	0	NULL	pan-caspase inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The pan-caspase inhibitor , z-VAD , prevents AICD in Th1 cells , but not Th2 cells , indicating different mechanisms of AICD in each T-helper subtype .
	manualset3
158089	2	411377	7	NULL	NULL	0	NULL	z-VAD 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The pan-caspase inhibitor , z-VAD , prevents AICD in Th1 cells , but not Th2 cells , indicating different mechanisms of AICD in each T-helper subtype .
	manualset3
158090	3	411377	7	NULL	NULL	0	NULL	AICD	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The pan-caspase inhibitor , z-VAD , prevents AICD in Th1 cells , but not Th2 cells , indicating different mechanisms of AICD in each T-helper subtype .
	manualset3
158091	4	411377	7	NULL	NULL	0	NULL	Th1 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The pan-caspase inhibitor , z-VAD , prevents AICD in Th1 cells , but not Th2 cells , indicating different mechanisms of AICD in each T-helper subtype .
	manualset3
158092	5	411377	7	NULL	NULL	0	NULL	Th2 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The pan-caspase inhibitor , z-VAD , prevents AICD in Th1 cells , but not Th2 cells , indicating different mechanisms of AICD in each T-helper subtype .
	manualset3
158093	6	411377	7	NULL	NULL	0	NULL	AICD	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The pan-caspase inhibitor , z-VAD , prevents AICD in Th1 cells , but not Th2 cells , indicating different mechanisms of AICD in each T-helper subtype .
	manualset3
158094	7	411377	7	NULL	NULL	0	NULL	T-helper subtype	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The pan-caspase inhibitor , z-VAD , prevents AICD in Th1 cells , but not Th2 cells , indicating different mechanisms of AICD in each T-helper subtype .
	manualset3
158521	8	411377	7	NULL	NULL	0	NULL	mechanisms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The pan-caspase inhibitor , z-VAD , prevents AICD in Th1 cells , but not Th2 cells , indicating different mechanisms of AICD in each T-helper subtype .
	manualset3
158095	1	411378	7	NULL	NULL	NULL	NULL	Clinical pictures	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Clinical pictures of pulmonary aspergillosis ) .
	manualset3
158096	2	411378	7	NULL	NULL	NULL	NULL	pulmonary aspergillosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Clinical pictures of pulmonary aspergillosis ) .
	manualset3
158097	1	411379	7	NULL	NULL	0	NULL	ADAMTS13	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	ADAMTS13 is a metalloproteinase that cleaves von Willebrand factor ( VWF ) multimers .
	manualset3
158098	2	411379	7	NULL	NULL	0	NULL	metalloproteinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	ADAMTS13 is a metalloproteinase that cleaves von Willebrand factor ( VWF ) multimers .
	manualset3
158099	3	411379	7	NULL	NULL	0	NULL	 von Willebrand factor ( VWF ) multimers	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	ADAMTS13 is a metalloproteinase that cleaves von Willebrand factor ( VWF ) multimers .
	manualset3
158100	1	411380	7	NULL	NULL	0	NULL	pancreas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The pancreas was intraductally distended with Liberase PI enzyme and normothermically digested .
	manualset3
158101	2	411380	7	NULL	NULL	0	NULL	Liberase PI enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The pancreas was intraductally distended with Liberase PI enzyme and normothermically digested .
	manualset3
158522	3	411380	7	NULL	NULL	0	NULL	normothermically digested 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The pancreas was intraductally distended with Liberase PI enzyme and normothermically digested .
	manualset3
158102	1	411381	7	NULL	NULL	0	NULL	pancreatic duct-epithelium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The pancreatic duct-epithelium has been considering as a pool of pancreatic stem/progenitor cells , cytokeratin-19 positive stem cells , which have been proved to be capable of differentiating into endocrine cells and inducing immune tolerance .
	manualset3
158103	2	411381	7	NULL	NULL	0	NULL	pool	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The pancreatic duct-epithelium has been considering as a pool of pancreatic stem/progenitor cells , cytokeratin-19 positive stem cells , which have been proved to be capable of differentiating into endocrine cells and inducing immune tolerance .
	manualset3
158104	3	411381	7	NULL	NULL	0	NULL	pancreatic stem/progenitor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The pancreatic duct-epithelium has been considering as a pool of pancreatic stem/progenitor cells , cytokeratin-19 positive stem cells , which have been proved to be capable of differentiating into endocrine cells and inducing immune tolerance .
	manualset3
158105	4	411381	7	NULL	NULL	0	NULL	cytokeratin-19 positive stem cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The pancreatic duct-epithelium has been considering as a pool of pancreatic stem/progenitor cells , cytokeratin-19 positive stem cells , which have been proved to be capable of differentiating into endocrine cells and inducing immune tolerance .
	manualset3
158106	5	411381	7	NULL	NULL	0	NULL	endocrine cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The pancreatic duct-epithelium has been considering as a pool of pancreatic stem/progenitor cells , cytokeratin-19 positive stem cells , which have been proved to be capable of differentiating into endocrine cells and inducing immune tolerance .
	manualset3
158107	6	411381	7	NULL	NULL	0	NULL	immune tolerance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The pancreatic duct-epithelium has been considering as a pool of pancreatic stem/progenitor cells , cytokeratin-19 positive stem cells , which have been proved to be capable of differentiating into endocrine cells and inducing immune tolerance .
	manualset3
158108	1	411382	7	NULL	NULL	0	NULL	 paper 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper also enlighten the scope of strengthening the existing system , by effectively training the existing workforce for their capacity building , and highlights training opportunities for working professional to pursue a related academic program .
	manualset3
158109	2	411382	7	NULL	NULL	0	NULL	scope	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper also enlighten the scope of strengthening the existing system , by effectively training the existing workforce for their capacity building , and highlights training opportunities for working professional to pursue a related academic program .
	manualset3
158110	3	411382	7	NULL	NULL	0	NULL	existing system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper also enlighten the scope of strengthening the existing system , by effectively training the existing workforce for their capacity building , and highlights training opportunities for working professional to pursue a related academic program .
	manualset3
158111	4	411382	7	NULL	NULL	NULL	NULL	workforce 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The paper also enlighten the scope of strengthening the existing system , by effectively training the existing workforce for their capacity building , and highlights training opportunities for working professional to pursue a related academic program .
	manualset3
158112	5	411382	7	NULL	NULL	0	NULL	capacity building	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper also enlighten the scope of strengthening the existing system , by effectively training the existing workforce for their capacity building , and highlights training opportunities for working professional to pursue a related academic program .
	manualset3
158113	6	411382	7	NULL	NULL	0	NULL	opportunities	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper also enlighten the scope of strengthening the existing system , by effectively training the existing workforce for their capacity building , and highlights training opportunities for working professional to pursue a related academic program .
	manualset3
158114	7	411382	7	NULL	NULL	0	NULL	working professional	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper also enlighten the scope of strengthening the existing system , by effectively training the existing workforce for their capacity building , and highlights training opportunities for working professional to pursue a related academic program .
	manualset3
158115	8	411382	7	NULL	NULL	0	NULL	academic program	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper also enlighten the scope of strengthening the existing system , by effectively training the existing workforce for their capacity building , and highlights training opportunities for working professional to pursue a related academic program .
	manualset3
158116	1	411383	7	NULL	NULL	0	NULL	paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper comes to several conclusions .
	manualset3
158117	2	411383	7	NULL	NULL	0	NULL	conclusions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper comes to several conclusions .
	manualset3
158118	1	411384	7	NULL	NULL	0	NULL	 paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper concludes that research that identifies and quantifies the public health factors of gambling will substantially contribute to a public shift toward a public health frame .
	manualset3
158119	2	411384	7	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper concludes that research that identifies and quantifies the public health factors of gambling will substantially contribute to a public shift toward a public health frame .
	manualset3
158120	3	411384	7	NULL	NULL	0	NULL	public health factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper concludes that research that identifies and quantifies the public health factors of gambling will substantially contribute to a public shift toward a public health frame .
	manualset3
158121	4	411384	7	NULL	NULL	0	NULL	gambling	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper concludes that research that identifies and quantifies the public health factors of gambling will substantially contribute to a public shift toward a public health frame .
	manualset3
158122	5	411384	7	NULL	NULL	0	NULL	public shift 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper concludes that research that identifies and quantifies the public health factors of gambling will substantially contribute to a public shift toward a public health frame .
	manualset3
158123	6	411384	7	NULL	NULL	0	NULL	public health frame	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper concludes that research that identifies and quantifies the public health factors of gambling will substantially contribute to a public shift toward a public health frame .
	manualset3
158124	1	411385	7	NULL	NULL	0	NULL	 paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper highlights the need for methodological rigor in study design , and the careful selection of appropriate , sensitive , reliable and clinically meaningful outcome measures to evaluate the impact of post-operative arm morbidity .
	manualset3
158125	2	411385	7	NULL	NULL	0	NULL	 methodological rigor	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper highlights the need for methodological rigor in study design , and the careful selection of appropriate , sensitive , reliable and clinically meaningful outcome measures to evaluate the impact of post-operative arm morbidity .
	manualset3
158126	3	411385	7	NULL	NULL	0	NULL	study design	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper highlights the need for methodological rigor in study design , and the careful selection of appropriate , sensitive , reliable and clinically meaningful outcome measures to evaluate the impact of post-operative arm morbidity .
	manualset3
158127	4	411385	7	NULL	NULL	0	NULL	careful selection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper highlights the need for methodological rigor in study design , and the careful selection of appropriate , sensitive , reliable and clinically meaningful outcome measures to evaluate the impact of post-operative arm morbidity .
	manualset3
158128	5	411385	7	NULL	NULL	0	NULL	clinically meaningful outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper highlights the need for methodological rigor in study design , and the careful selection of appropriate , sensitive , reliable and clinically meaningful outcome measures to evaluate the impact of post-operative arm morbidity .
	manualset3
158129	6	411385	7	NULL	NULL	0	NULL	impact 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper highlights the need for methodological rigor in study design , and the careful selection of appropriate , sensitive , reliable and clinically meaningful outcome measures to evaluate the impact of post-operative arm morbidity .
	manualset3
158130	7	411385	7	NULL	NULL	0	NULL	post-operative arm morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper highlights the need for methodological rigor in study design , and the careful selection of appropriate , sensitive , reliable and clinically meaningful outcome measures to evaluate the impact of post-operative arm morbidity .
	manualset3
158131	8	411385	7	NULL	NULL	0	NULL	need	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper highlights the need for methodological rigor in study design , and the careful selection of appropriate , sensitive , reliable and clinically meaningful outcome measures to evaluate the impact of post-operative arm morbidity .
	manualset3
158132	1	411386	7	NULL	NULL	0	NULL	paper 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper is the result of five years paediatric , neurological and neurosurgical care of 102 infants with inborn and acquired damage of the central nervous system .
	manualset3
158133	2	411386	7	NULL	NULL	0	NULL	result 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper is the result of five years paediatric , neurological and neurosurgical care of 102 infants with inborn and acquired damage of the central nervous system .
	manualset3
158134	3	411386	7	NULL	NULL	0	NULL	 five years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper is the result of five years paediatric , neurological and neurosurgical care of 102 infants with inborn and acquired damage of the central nervous system .
	manualset3
158135	4	411386	7	NULL	NULL	0	NULL	paediatric care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper is the result of five years paediatric , neurological and neurosurgical care of 102 infants with inborn and acquired damage of the central nervous system .
	manualset3
158136	5	411386	7	NULL	NULL	0	NULL	neurological care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper is the result of five years paediatric , neurological and neurosurgical care of 102 infants with inborn and acquired damage of the central nervous system .
	manualset3
158137	6	411386	7	NULL	NULL	0	NULL	neurosurgical care 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper is the result of five years paediatric , neurological and neurosurgical care of 102 infants with inborn and acquired damage of the central nervous system .
	manualset3
158138	7	411386	7	NULL	NULL	0	NULL	102 infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper is the result of five years paediatric , neurological and neurosurgical care of 102 infants with inborn and acquired damage of the central nervous system .
	manualset3
158139	8	411386	7	NULL	NULL	NULL	NULL	inborn damage	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The paper is the result of five years paediatric , neurological and neurosurgical care of 102 infants with inborn and acquired damage of the central nervous system .
	manualset3
158140	9	411386	7	NULL	NULL	NULL	NULL	acquired damage	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The paper is the result of five years paediatric , neurological and neurosurgical care of 102 infants with inborn and acquired damage of the central nervous system .
	manualset3
158141	10	411386	7	NULL	NULL	0	NULL	central nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper is the result of five years paediatric , neurological and neurosurgical care of 102 infants with inborn and acquired damage of the central nervous system .
	manualset3
158142	1	411387	7	NULL	NULL	0	NULL	paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper looks at how ESTAMOS ( a Mozambican NGO ) and WaterAid introduced EcoSan in Lichinga , how families and communities have responded to EcoSan , and key lessons learned during the process to date that could be relevant to others within and beyond Mozambique .
	manualset3
158143	2	411387	7	NULL	NULL	0	NULL	ESTAMOS ( a Mozambican NGO )	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper looks at how ESTAMOS ( a Mozambican NGO ) and WaterAid introduced EcoSan in Lichinga , how families and communities have responded to EcoSan , and key lessons learned during the process to date that could be relevant to others within and beyond Mozambique .
	manualset3
158144	3	411387	7	NULL	NULL	0	NULL	WaterAid introduced EcoSan	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper looks at how ESTAMOS ( a Mozambican NGO ) and WaterAid introduced EcoSan in Lichinga , how families and communities have responded to EcoSan , and key lessons learned during the process to date that could be relevant to others within and beyond Mozambique .
	manualset3
158145	4	411387	7	NULL	NULL	0	NULL	Lichinga	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper looks at how ESTAMOS ( a Mozambican NGO ) and WaterAid introduced EcoSan in Lichinga , how families and communities have responded to EcoSan , and key lessons learned during the process to date that could be relevant to others within and beyond Mozambique .
	manualset3
158146	5	411387	7	NULL	NULL	NULL	NULL	families	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The paper looks at how ESTAMOS ( a Mozambican NGO ) and WaterAid introduced EcoSan in Lichinga , how families and communities have responded to EcoSan , and key lessons learned during the process to date that could be relevant to others within and beyond Mozambique .
	manualset3
158147	6	411387	7	NULL	NULL	NULL	NULL	communities	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The paper looks at how ESTAMOS ( a Mozambican NGO ) and WaterAid introduced EcoSan in Lichinga , how families and communities have responded to EcoSan , and key lessons learned during the process to date that could be relevant to others within and beyond Mozambique .
	manualset3
158148	7	411387	7	NULL	NULL	0	NULL	EcoSan	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper looks at how ESTAMOS ( a Mozambican NGO ) and WaterAid introduced EcoSan in Lichinga , how families and communities have responded to EcoSan , and key lessons learned during the process to date that could be relevant to others within and beyond Mozambique .
	manualset3
158149	8	411387	7	NULL	NULL	0	NULL	key lessons	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper looks at how ESTAMOS ( a Mozambican NGO ) and WaterAid introduced EcoSan in Lichinga , how families and communities have responded to EcoSan , and key lessons learned during the process to date that could be relevant to others within and beyond Mozambique .
	manualset3
158150	9	411387	7	NULL	NULL	0	NULL	process 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper looks at how ESTAMOS ( a Mozambican NGO ) and WaterAid introduced EcoSan in Lichinga , how families and communities have responded to EcoSan , and key lessons learned during the process to date that could be relevant to others within and beyond Mozambique .
	manualset3
158151	10	411387	7	NULL	NULL	0	NULL	date	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper looks at how ESTAMOS ( a Mozambican NGO ) and WaterAid introduced EcoSan in Lichinga , how families and communities have responded to EcoSan , and key lessons learned during the process to date that could be relevant to others within and beyond Mozambique .
	manualset3
158153	12	411387	7	NULL	NULL	0	NULL	Mozambique	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper looks at how ESTAMOS ( a Mozambican NGO ) and WaterAid introduced EcoSan in Lichinga , how families and communities have responded to EcoSan , and key lessons learned during the process to date that could be relevant to others within and beyond Mozambique .
	manualset3
158154	1	411388	7	NULL	NULL	0	NULL	paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper points the risks of understanding and misunderstanding - supervised training with practicing inside the dental school , under the label of curricular supervised training .
	manualset3
158155	2	411388	7	NULL	NULL	NULL	NULL	risks of understanding and misunderstanding	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The paper points the risks of understanding and misunderstanding - supervised training with practicing inside the dental school , under the label of curricular supervised training .
	manualset3
158156	4	411388	7	NULL	NULL	NULL	NULL	dental school	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The paper points the risks of understanding and misunderstanding - supervised training with practicing inside the dental school , under the label of curricular supervised training .
	manualset3
158157	5	411388	7	NULL	NULL	NULL	NULL	 label	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The paper points the risks of understanding and misunderstanding - supervised training with practicing inside the dental school , under the label of curricular supervised training .
	manualset3
158158	6	411388	7	NULL	NULL	NULL	NULL	curricular supervised training	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The paper points the risks of understanding and misunderstanding - supervised training with practicing inside the dental school , under the label of curricular supervised training .
	manualset3
158159	3	411388	7	NULL	NULL	NULL	NULL	supervised training	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The paper points the risks of understanding and misunderstanding - supervised training with practicing inside the dental school , under the label of curricular supervised training .
	manualset3
158160	1	411389	7	NULL	NULL	0	NULL	ADM	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	ADM and UK were infused in three different ways through the left gastric artery on laparotomy , that is , a mixture of both in the first group , ADM followed by UK in the second group and ADM after UK in the third group .
	manualset3
158161	2	411389	7	NULL	NULL	0	NULL	UK	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	ADM and UK were infused in three different ways through the left gastric artery on laparotomy , that is , a mixture of both in the first group , ADM followed by UK in the second group and ADM after UK in the third group .
	manualset3
158162	3	411389	7	NULL	NULL	0	NULL	three different ways	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	ADM and UK were infused in three different ways through the left gastric artery on laparotomy , that is , a mixture of both in the first group , ADM followed by UK in the second group and ADM after UK in the third group .
	manualset3
158163	4	411389	7	NULL	NULL	0	NULL	 left gastric artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	ADM and UK were infused in three different ways through the left gastric artery on laparotomy , that is , a mixture of both in the first group , ADM followed by UK in the second group and ADM after UK in the third group .
	manualset3
158164	5	411389	7	NULL	NULL	0	NULL	laparotomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	ADM and UK were infused in three different ways through the left gastric artery on laparotomy , that is , a mixture of both in the first group , ADM followed by UK in the second group and ADM after UK in the third group .
	manualset3
158165	6	411389	7	NULL	NULL	0	NULL	mixture	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	ADM and UK were infused in three different ways through the left gastric artery on laparotomy , that is , a mixture of both in the first group , ADM followed by UK in the second group and ADM after UK in the third group .
	manualset3
158166	7	411389	7	NULL	NULL	0	NULL	first group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	ADM and UK were infused in three different ways through the left gastric artery on laparotomy , that is , a mixture of both in the first group , ADM followed by UK in the second group and ADM after UK in the third group .
	manualset3
158167	8	411389	7	NULL	NULL	0	NULL	ADM	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	ADM and UK were infused in three different ways through the left gastric artery on laparotomy , that is , a mixture of both in the first group , ADM followed by UK in the second group and ADM after UK in the third group .
	manualset3
158168	9	411389	7	NULL	NULL	0	NULL	UK	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	ADM and UK were infused in three different ways through the left gastric artery on laparotomy , that is , a mixture of both in the first group , ADM followed by UK in the second group and ADM after UK in the third group .
	manualset3
158169	10	411389	7	NULL	NULL	0	NULL	second group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	ADM and UK were infused in three different ways through the left gastric artery on laparotomy , that is , a mixture of both in the first group , ADM followed by UK in the second group and ADM after UK in the third group .
	manualset3
158170	11	411389	7	NULL	NULL	0	NULL	ADM	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	ADM and UK were infused in three different ways through the left gastric artery on laparotomy , that is , a mixture of both in the first group , ADM followed by UK in the second group and ADM after UK in the third group .
	manualset3
158171	12	411389	7	NULL	NULL	0	NULL	UK 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	ADM and UK were infused in three different ways through the left gastric artery on laparotomy , that is , a mixture of both in the first group , ADM followed by UK in the second group and ADM after UK in the third group .
	manualset3
158172	13	411389	7	NULL	NULL	0	NULL	third group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	ADM and UK were infused in three different ways through the left gastric artery on laparotomy , that is , a mixture of both in the first group , ADM followed by UK in the second group and ADM after UK in the third group .
	manualset3
158173	1	411390	7	NULL	NULL	0	NULL	paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper presents the position that Freud was not torn by the conflict `` To be or not to be a Jew '' as some have contended , but , rather , that he had resolved upon `` to be ... '' , and did not long to reject his Jewish identity .
	manualset3
158174	2	411390	7	NULL	NULL	NULL	NULL	position	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The paper presents the position that Freud was not torn by the conflict `` To be or not to be a Jew '' as some have contended , but , rather , that he had resolved upon `` to be ... '' , and did not long to reject his Jewish identity .
	manualset3
158175	3	411390	7	NULL	NULL	NULL	NULL	Freud	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The paper presents the position that Freud was not torn by the conflict `` To be or not to be a Jew '' as some have contended , but , rather , that he had resolved upon `` to be ... '' , and did not long to reject his Jewish identity .
	manualset3
158176	4	411390	7	NULL	NULL	0	NULL	conflict	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper presents the position that Freud was not torn by the conflict `` To be or not to be a Jew '' as some have contended , but , rather , that he had resolved upon `` to be ... '' , and did not long to reject his Jewish identity .
	manualset3
158177	5	411390	7	NULL	NULL	0	NULL	 `` To be or not to be a Jew ''	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper presents the position that Freud was not torn by the conflict `` To be or not to be a Jew '' as some have contended , but , rather , that he had resolved upon `` to be ... '' , and did not long to reject his Jewish identity .
	manualset3
158178	6	411390	7	NULL	NULL	0	NULL	`` to be ... '	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper presents the position that Freud was not torn by the conflict `` To be or not to be a Jew '' as some have contended , but , rather , that he had resolved upon `` to be ... '' , and did not long to reject his Jewish identity .
	manualset3
158179	7	411390	7	NULL	NULL	0	NULL	Jewish identity	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper presents the position that Freud was not torn by the conflict `` To be or not to be a Jew '' as some have contended , but , rather , that he had resolved upon `` to be ... '' , and did not long to reject his Jewish identity .
	manualset3
158180	1	411391	7	NULL	NULL	0	NULL	paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper provides the results of studies of the impact of temperature on the structural and energetic state of drinking water and shows that the altered temperature conditions of water causes a change in its supramolecular structure and biological value .
	manualset3
158181	2	411391	7	NULL	NULL	0	NULL	results of studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper provides the results of studies of the impact of temperature on the structural and energetic state of drinking water and shows that the altered temperature conditions of water causes a change in its supramolecular structure and biological value .
	manualset3
158182	3	411391	7	NULL	NULL	0	NULL	impact of temperature	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper provides the results of studies of the impact of temperature on the structural and energetic state of drinking water and shows that the altered temperature conditions of water causes a change in its supramolecular structure and biological value .
	manualset3
158183	4	411391	7	NULL	NULL	0	NULL	structural  state of drinking water	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper provides the results of studies of the impact of temperature on the structural and energetic state of drinking water and shows that the altered temperature conditions of water causes a change in its supramolecular structure and biological value .
	manualset3
158184	5	411391	7	NULL	NULL	0	NULL	energetic state of drinking water	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper provides the results of studies of the impact of temperature on the structural and energetic state of drinking water and shows that the altered temperature conditions of water causes a change in its supramolecular structure and biological value .
	manualset3
158185	6	411391	7	NULL	NULL	0	NULL	 altered temperature conditions	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper provides the results of studies of the impact of temperature on the structural and energetic state of drinking water and shows that the altered temperature conditions of water causes a change in its supramolecular structure and biological value .
	manualset3
158186	7	411391	7	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper provides the results of studies of the impact of temperature on the structural and energetic state of drinking water and shows that the altered temperature conditions of water causes a change in its supramolecular structure and biological value .
	manualset3
158187	8	411391	7	NULL	NULL	0	NULL	change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper provides the results of studies of the impact of temperature on the structural and energetic state of drinking water and shows that the altered temperature conditions of water causes a change in its supramolecular structure and biological value .
	manualset3
158188	9	411391	7	NULL	NULL	NULL	NULL	supramolecular structure	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The paper provides the results of studies of the impact of temperature on the structural and energetic state of drinking water and shows that the altered temperature conditions of water causes a change in its supramolecular structure and biological value .
	manualset3
158189	10	411391	7	NULL	NULL	0	NULL	biological value	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper provides the results of studies of the impact of temperature on the structural and energetic state of drinking water and shows that the altered temperature conditions of water causes a change in its supramolecular structure and biological value .
	manualset3
158190	1	411392	7	NULL	NULL	NULL	NULL	paradox	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The paradox of transferrin receptor-mediated drug delivery -- intracellular targeting or transcellular transport ?
	manualset3
158191	2	411392	7	NULL	NULL	0	NULL	transferrin receptor-mediated drug delivery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The paradox of transferrin receptor-mediated drug delivery -- intracellular targeting or transcellular transport ?
	manualset3
158192	3	411392	7	NULL	NULL	0	NULL	 intracellular targeting	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The paradox of transferrin receptor-mediated drug delivery -- intracellular targeting or transcellular transport ?
	manualset3
158193	4	411392	7	NULL	NULL	0	NULL	transcellular transport	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The paradox of transferrin receptor-mediated drug delivery -- intracellular targeting or transcellular transport ?
	manualset3
158194	1	411393	7	NULL	NULL	NULL	NULL	parameters of the prisms	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The parameters of the prisms , particularly their angles , are studied to improve the design , and we demonstrate the maximum attenuation range that this type of attenuator can provide .
	manualset3
158195	2	411393	7	NULL	NULL	NULL	NULL	angles	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The parameters of the prisms , particularly their angles , are studied to improve the design , and we demonstrate the maximum attenuation range that this type of attenuator can provide .
	manualset3
158196	3	411393	7	NULL	NULL	0	NULL	design	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The parameters of the prisms , particularly their angles , are studied to improve the design , and we demonstrate the maximum attenuation range that this type of attenuator can provide .
	manualset3
158197	4	411393	7	NULL	NULL	0	NULL	maximum attenuation range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The parameters of the prisms , particularly their angles , are studied to improve the design , and we demonstrate the maximum attenuation range that this type of attenuator can provide .
	manualset3
158198	5	411393	7	NULL	NULL	0	NULL	attenuator	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The parameters of the prisms , particularly their angles , are studied to improve the design , and we demonstrate the maximum attenuation range that this type of attenuator can provide .
	manualset3
158199	1	411394	7	NULL	NULL	0	NULL	 parameters	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The parameters used to evaluate the process of wound healing of these incisions were the assay of type-I collagen , type-III collagen ( procollagen peptide PIPC and P III P , each being the precursor of collagen ) , type-IV collagen , and hydroxyproline .
	manualset3
158200	2	411394	7	NULL	NULL	NULL	NULL	process	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The parameters used to evaluate the process of wound healing of these incisions were the assay of type-I collagen , type-III collagen ( procollagen peptide PIPC and P III P , each being the precursor of collagen ) , type-IV collagen , and hydroxyproline .
	manualset3
158201	3	411394	7	NULL	NULL	0	NULL	wound healing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The parameters used to evaluate the process of wound healing of these incisions were the assay of type-I collagen , type-III collagen ( procollagen peptide PIPC and P III P , each being the precursor of collagen ) , type-IV collagen , and hydroxyproline .
	manualset3
158202	4	411394	7	NULL	NULL	0	NULL	 incisions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The parameters used to evaluate the process of wound healing of these incisions were the assay of type-I collagen , type-III collagen ( procollagen peptide PIPC and P III P , each being the precursor of collagen ) , type-IV collagen , and hydroxyproline .
	manualset3
158203	5	411394	7	NULL	NULL	0	NULL	assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The parameters used to evaluate the process of wound healing of these incisions were the assay of type-I collagen , type-III collagen ( procollagen peptide PIPC and P III P , each being the precursor of collagen ) , type-IV collagen , and hydroxyproline .
	manualset3
158204	6	411394	7	NULL	NULL	0	NULL	type-I collagen 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The parameters used to evaluate the process of wound healing of these incisions were the assay of type-I collagen , type-III collagen ( procollagen peptide PIPC and P III P , each being the precursor of collagen ) , type-IV collagen , and hydroxyproline .
	manualset3
158205	7	411394	7	NULL	NULL	0	NULL	type-III collagen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The parameters used to evaluate the process of wound healing of these incisions were the assay of type-I collagen , type-III collagen ( procollagen peptide PIPC and P III P , each being the precursor of collagen ) , type-IV collagen , and hydroxyproline .
	manualset3
158206	8	411394	7	NULL	NULL	0	NULL	procollagen peptide PIPC	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The parameters used to evaluate the process of wound healing of these incisions were the assay of type-I collagen , type-III collagen ( procollagen peptide PIPC and P III P , each being the precursor of collagen ) , type-IV collagen , and hydroxyproline .
	manualset3
158207	9	411394	7	NULL	NULL	0	NULL	P III P 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The parameters used to evaluate the process of wound healing of these incisions were the assay of type-I collagen , type-III collagen ( procollagen peptide PIPC and P III P , each being the precursor of collagen ) , type-IV collagen , and hydroxyproline .
	manualset3
158208	10	411394	7	NULL	NULL	0	NULL	precursor of collagen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The parameters used to evaluate the process of wound healing of these incisions were the assay of type-I collagen , type-III collagen ( procollagen peptide PIPC and P III P , each being the precursor of collagen ) , type-IV collagen , and hydroxyproline .
	manualset3
158209	11	411394	7	NULL	NULL	0	NULL	type-IV collagen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The parameters used to evaluate the process of wound healing of these incisions were the assay of type-I collagen , type-III collagen ( procollagen peptide PIPC and P III P , each being the precursor of collagen ) , type-IV collagen , and hydroxyproline .
	manualset3
158210	12	411394	7	NULL	NULL	0	NULL	hydroxyproline	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The parameters used to evaluate the process of wound healing of these incisions were the assay of type-I collagen , type-III collagen ( procollagen peptide PIPC and P III P , each being the precursor of collagen ) , type-IV collagen , and hydroxyproline .
	manualset3
158211	1	411395	7	NULL	NULL	0	NULL	ADMA	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	ADMA correlated with SDMA , L-arginine , and plasma creatinine ( all P & lt ; 0.05 ) but not with age , body mass index , D-dimer , thrombus extension , or history of symptoms .
	manualset3
158212	2	411395	7	NULL	NULL	0	NULL	SDMA	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	ADMA correlated with SDMA , L-arginine , and plasma creatinine ( all P & lt ; 0.05 ) but not with age , body mass index , D-dimer , thrombus extension , or history of symptoms .
	manualset3
158213	3	411395	7	NULL	NULL	0	NULL	L-arginine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	ADMA correlated with SDMA , L-arginine , and plasma creatinine ( all P & lt ; 0.05 ) but not with age , body mass index , D-dimer , thrombus extension , or history of symptoms .
	manualset3
158214	4	411395	7	NULL	NULL	0	NULL	 plasma creatinine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	ADMA correlated with SDMA , L-arginine , and plasma creatinine ( all P & lt ; 0.05 ) but not with age , body mass index , D-dimer , thrombus extension , or history of symptoms .
	manualset3
158215	5	411395	7	NULL	NULL	0	NULL	all P & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	ADMA correlated with SDMA , L-arginine , and plasma creatinine ( all P & lt ; 0.05 ) but not with age , body mass index , D-dimer , thrombus extension , or history of symptoms .
	manualset3
158216	6	411395	7	NULL	NULL	NULL	NULL	age	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ADMA correlated with SDMA , L-arginine , and plasma creatinine ( all P & lt ; 0.05 ) but not with age , body mass index , D-dimer , thrombus extension , or history of symptoms .
	manualset3
158217	7	411395	7	NULL	NULL	0	NULL	body mass index	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	ADMA correlated with SDMA , L-arginine , and plasma creatinine ( all P & lt ; 0.05 ) but not with age , body mass index , D-dimer , thrombus extension , or history of symptoms .
	manualset3
158218	8	411395	7	NULL	NULL	NULL	NULL	D-dimer	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ADMA correlated with SDMA , L-arginine , and plasma creatinine ( all P & lt ; 0.05 ) but not with age , body mass index , D-dimer , thrombus extension , or history of symptoms .
	manualset3
158219	9	411395	7	NULL	NULL	NULL	NULL	thrombus extension	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ADMA correlated with SDMA , L-arginine , and plasma creatinine ( all P & lt ; 0.05 ) but not with age , body mass index , D-dimer , thrombus extension , or history of symptoms .
	manualset3
158220	10	411395	7	NULL	NULL	0	NULL	history of symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	ADMA correlated with SDMA , L-arginine , and plasma creatinine ( all P & lt ; 0.05 ) but not with age , body mass index , D-dimer , thrombus extension , or history of symptoms .
	manualset3
158221	1	411396	7	NULL	NULL	0	NULL	parapharyngeal section of cartilaginous ET	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The parapharyngeal section of cartilaginous ET , however , was found to include an open lumen , where pulsatile movements of the medioinferior membranous ET wall could be seen .
	manualset3
158222	2	411396	7	NULL	NULL	0	NULL	open lumen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The parapharyngeal section of cartilaginous ET , however , was found to include an open lumen , where pulsatile movements of the medioinferior membranous ET wall could be seen .
	manualset3
158223	3	411396	7	NULL	NULL	0	NULL	pulsatile movements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The parapharyngeal section of cartilaginous ET , however , was found to include an open lumen , where pulsatile movements of the medioinferior membranous ET wall could be seen .
	manualset3
158224	4	411396	7	NULL	NULL	0	NULL	medioinferior membranous ET wall	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The parapharyngeal section of cartilaginous ET , however , was found to include an open lumen , where pulsatile movements of the medioinferior membranous ET wall could be seen .
	manualset3
158225	1	411397	7	NULL	NULL	0	NULL	parasite	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The parasite , once phagocytosed by the hemocyte , the main cellular effector of the immune system , appears to have some counter mechanism that turns off the haemocyte 's metabolic destructive capacity , so that the parasite survives within the cell .
	manualset3
158226	2	411397	7	NULL	NULL	NULL	NULL	 hemocyte	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The parasite , once phagocytosed by the hemocyte , the main cellular effector of the immune system , appears to have some counter mechanism that turns off the haemocyte 's metabolic destructive capacity , so that the parasite survives within the cell .
	manualset3
158227	3	411397	7	NULL	NULL	NULL	NULL	cellular effector	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The parasite , once phagocytosed by the hemocyte , the main cellular effector of the immune system , appears to have some counter mechanism that turns off the haemocyte 's metabolic destructive capacity , so that the parasite survives within the cell .
	manualset3
158228	4	411397	7	NULL	NULL	0	NULL	immune system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The parasite , once phagocytosed by the hemocyte , the main cellular effector of the immune system , appears to have some counter mechanism that turns off the haemocyte 's metabolic destructive capacity , so that the parasite survives within the cell .
	manualset3
158229	5	411397	7	NULL	NULL	0	NULL	counter mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The parasite , once phagocytosed by the hemocyte , the main cellular effector of the immune system , appears to have some counter mechanism that turns off the haemocyte 's metabolic destructive capacity , so that the parasite survives within the cell .
	manualset3
158230	6	411397	7	NULL	NULL	0	NULL	haemocyte 's metabolic destructive capacity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The parasite , once phagocytosed by the hemocyte , the main cellular effector of the immune system , appears to have some counter mechanism that turns off the haemocyte 's metabolic destructive capacity , so that the parasite survives within the cell .
	manualset3
158231	7	411397	7	NULL	NULL	0	NULL	parasite	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The parasite , once phagocytosed by the hemocyte , the main cellular effector of the immune system , appears to have some counter mechanism that turns off the haemocyte 's metabolic destructive capacity , so that the parasite survives within the cell .
	manualset3
158232	8	411397	7	NULL	NULL	0	NULL	cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The parasite , once phagocytosed by the hemocyte , the main cellular effector of the immune system , appears to have some counter mechanism that turns off the haemocyte 's metabolic destructive capacity , so that the parasite survives within the cell .
	manualset3
158233	1	411398	7	NULL	NULL	0	NULL	parent RIC ( TM negative ) line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The parent RIC ( TM negative ) line responded to alpha-thrombin and to agonist peptide ( SFLLRN-PNDKYEPF ; abbreviated SFLL ) with both mitogenic response and phosphoinositol release .
	manualset3
158234	2	411398	7	NULL	NULL	0	NULL	alpha-thrombin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The parent RIC ( TM negative ) line responded to alpha-thrombin and to agonist peptide ( SFLLRN-PNDKYEPF ; abbreviated SFLL ) with both mitogenic response and phosphoinositol release .
	manualset3
158235	3	411398	7	NULL	NULL	0	NULL	agonist peptide ( SFLLRN-PNDKYEPF ; abbreviated SFLL )	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The parent RIC ( TM negative ) line responded to alpha-thrombin and to agonist peptide ( SFLLRN-PNDKYEPF ; abbreviated SFLL ) with both mitogenic response and phosphoinositol release .
	manualset3
158236	4	411398	7	NULL	NULL	NULL	NULL	mitogenic response	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The parent RIC ( TM negative ) line responded to alpha-thrombin and to agonist peptide ( SFLLRN-PNDKYEPF ; abbreviated SFLL ) with both mitogenic response and phosphoinositol release .
	manualset3
158237	5	411398	7	NULL	NULL	NULL	NULL	phosphoinositol release 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The parent RIC ( TM negative ) line responded to alpha-thrombin and to agonist peptide ( SFLLRN-PNDKYEPF ; abbreviated SFLL ) with both mitogenic response and phosphoinositol release .
	manualset3
158238	1	411399	7	NULL	NULL	0	NULL	parental strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The parental strains were virulent , inducing severe diarrhoea , dehydration and systemic disease .
	manualset3
158239	2	411399	7	NULL	NULL	0	NULL	virulent	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The parental strains were virulent , inducing severe diarrhoea , dehydration and systemic disease .
	manualset3
158240	3	411399	7	NULL	NULL	0	NULL	severe diarrhoea	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The parental strains were virulent , inducing severe diarrhoea , dehydration and systemic disease .
	manualset3
158241	4	411399	7	NULL	NULL	0	NULL	dehydration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The parental strains were virulent , inducing severe diarrhoea , dehydration and systemic disease .
	manualset3
158242	5	411399	7	NULL	NULL	0	NULL	systemic disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The parental strains were virulent , inducing severe diarrhoea , dehydration and systemic disease .
	manualset3
158243	1	411400	7	NULL	NULL	0	NULL	 partial characterization of the C1q receptor ( C1q-R ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The partial characterization and expression of the C1q receptor ( C1q-R ) in relation to other complement receptors present on the surface of neutrophils has been examined , as well as the effects of free C1q on cell function .
	manualset3
158244	2	411400	7	NULL	NULL	0	NULL	expression of the C1q receptor ( C1q-R )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The partial characterization and expression of the C1q receptor ( C1q-R ) in relation to other complement receptors present on the surface of neutrophils has been examined , as well as the effects of free C1q on cell function .
	manualset3
158245	3	411400	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The partial characterization and expression of the C1q receptor ( C1q-R ) in relation to other complement receptors present on the surface of neutrophils has been examined , as well as the effects of free C1q on cell function .
	manualset3
158246	4	411400	7	NULL	NULL	0	NULL	complement receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The partial characterization and expression of the C1q receptor ( C1q-R ) in relation to other complement receptors present on the surface of neutrophils has been examined , as well as the effects of free C1q on cell function .
	manualset3
158247	5	411400	7	NULL	NULL	0	NULL	surface of neutrophils	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The partial characterization and expression of the C1q receptor ( C1q-R ) in relation to other complement receptors present on the surface of neutrophils has been examined , as well as the effects of free C1q on cell function .
	manualset3
158248	6	411400	7	NULL	NULL	NULL	NULL	effects of free C1q 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The partial characterization and expression of the C1q receptor ( C1q-R ) in relation to other complement receptors present on the surface of neutrophils has been examined , as well as the effects of free C1q on cell function .
	manualset3
158250	7	411400	7	NULL	NULL	NULL	NULL	 cell function	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The partial characterization and expression of the C1q receptor ( C1q-R ) in relation to other complement receptors present on the surface of neutrophils has been examined , as well as the effects of free C1q on cell function .
	manualset3
158251	1	411401	7	NULL	NULL	NULL	NULL	partial eviction of H3	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The partial eviction of H3 from the nucleosomes is dependent on ubiquitinated H2A Lys-119 / Lys-120 .
	manualset3
158252	2	411401	7	NULL	NULL	0	NULL	nucleosomes 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The partial eviction of H3 from the nucleosomes is dependent on ubiquitinated H2A Lys-119 / Lys-120 .
	manualset3
158253	3	411401	7	NULL	NULL	0	NULL	ubiquitinated H2A Lys-119 / Lys-120	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The partial eviction of H3 from the nucleosomes is dependent on ubiquitinated H2A Lys-119 / Lys-120 .
	manualset3
158254	1	411402	7	NULL	NULL	0	NULL	participants in courses ( experimental group )	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The participants in courses ( experimental group ) , who according to their situation were supposed to have a substantial higher rate of recidivism , had an actual recidivism-rate , which was significantly lower than the rate of the control group .
	manualset3
158256	2	411402	7	NULL	NULL	NULL	NULL	situation	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The participants in courses ( experimental group ) , who according to their situation were supposed to have a substantial higher rate of recidivism , had an actual recidivism-rate , which was significantly lower than the rate of the control group .
	manualset3
158257	3	411402	7	NULL	NULL	0	NULL	recidivism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The participants in courses ( experimental group ) , who according to their situation were supposed to have a substantial higher rate of recidivism , had an actual recidivism-rate , which was significantly lower than the rate of the control group .
	manualset3
158258	4	411402	7	NULL	NULL	0	NULL	recidivism-rate 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The participants in courses ( experimental group ) , who according to their situation were supposed to have a substantial higher rate of recidivism , had an actual recidivism-rate , which was significantly lower than the rate of the control group .
	manualset3
158259	5	411402	7	NULL	NULL	0	NULL	control group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The participants in courses ( experimental group ) , who according to their situation were supposed to have a substantial higher rate of recidivism , had an actual recidivism-rate , which was significantly lower than the rate of the control group .
	manualset3
158525	6	411402	7	NULL	NULL	0	NULL	higher rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The participants in courses ( experimental group ) , who according to their situation were supposed to have a substantial higher rate of recidivism , had an actual recidivism-rate , which was significantly lower than the rate of the control group .
	manualset3
158526	7	411402	7	NULL	NULL	0	NULL	rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The participants in courses ( experimental group ) , who according to their situation were supposed to have a substantial higher rate of recidivism , had an actual recidivism-rate , which was significantly lower than the rate of the control group .
	manualset3
158260	1	411403	7	NULL	NULL	0	NULL	participation of DNA photolyase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The participation of DNA photolyase in dark repair processes has been reported in some heterotrophic organisms .
	manualset3
158261	2	411403	7	NULL	NULL	0	NULL	dark repair processes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The participation of DNA photolyase in dark repair processes has been reported in some heterotrophic organisms .
	manualset3
158262	3	411403	7	NULL	NULL	0	NULL	heterotrophic organisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The participation of DNA photolyase in dark repair processes has been reported in some heterotrophic organisms .
	manualset3
158263	1	411404	7	NULL	NULL	NULL	NULL	participation of microtubules	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The participation of microtubules in these movements is inferred from the observation that LSM cease after treatment with drugs which depolymerize microtubules , i.e. , colchicine , Vinblastine , and podophyllin .
	manualset3
158264	2	411404	7	NULL	NULL	0	NULL	movements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The participation of microtubules in these movements is inferred from the observation that LSM cease after treatment with drugs which depolymerize microtubules , i.e. , colchicine , Vinblastine , and podophyllin .
	manualset3
158265	3	411404	7	NULL	NULL	0	NULL	observation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The participation of microtubules in these movements is inferred from the observation that LSM cease after treatment with drugs which depolymerize microtubules , i.e. , colchicine , Vinblastine , and podophyllin .
	manualset3
158266	4	411404	7	NULL	NULL	0	NULL	LSM	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The participation of microtubules in these movements is inferred from the observation that LSM cease after treatment with drugs which depolymerize microtubules , i.e. , colchicine , Vinblastine , and podophyllin .
	manualset3
158267	5	411404	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The participation of microtubules in these movements is inferred from the observation that LSM cease after treatment with drugs which depolymerize microtubules , i.e. , colchicine , Vinblastine , and podophyllin .
	manualset3
158268	6	411404	7	NULL	NULL	0	NULL	drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The participation of microtubules in these movements is inferred from the observation that LSM cease after treatment with drugs which depolymerize microtubules , i.e. , colchicine , Vinblastine , and podophyllin .
	manualset3
158269	7	411404	7	NULL	NULL	0	NULL	depolymerize	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The participation of microtubules in these movements is inferred from the observation that LSM cease after treatment with drugs which depolymerize microtubules , i.e. , colchicine , Vinblastine , and podophyllin .
	manualset3
158270	8	411404	7	NULL	NULL	0	NULL	microtubules	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The participation of microtubules in these movements is inferred from the observation that LSM cease after treatment with drugs which depolymerize microtubules , i.e. , colchicine , Vinblastine , and podophyllin .
	manualset3
158271	9	411404	7	NULL	NULL	0	NULL	colchicine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The participation of microtubules in these movements is inferred from the observation that LSM cease after treatment with drugs which depolymerize microtubules , i.e. , colchicine , Vinblastine , and podophyllin .
	manualset3
158272	10	411404	7	NULL	NULL	0	NULL	Vinblastine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The participation of microtubules in these movements is inferred from the observation that LSM cease after treatment with drugs which depolymerize microtubules , i.e. , colchicine , Vinblastine , and podophyllin .
	manualset3
158273	11	411404	7	NULL	NULL	0	NULL	podophyllin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The participation of microtubules in these movements is inferred from the observation that LSM cease after treatment with drugs which depolymerize microtubules , i.e. , colchicine , Vinblastine , and podophyllin .
	manualset3
158274	1	411405	7	NULL	NULL	0	NULL	AE1/F ( c ) receptor chimeras	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	AE1/F ( c ) receptor chimeras have been used to define the sequences that direct the basolateral sorting , recycling and cytoskeletal association of the chicken AE1-4 anion exchanger in MDCK cells .
	manualset3
158275	2	411405	7	NULL	NULL	0	NULL	sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	AE1/F ( c ) receptor chimeras have been used to define the sequences that direct the basolateral sorting , recycling and cytoskeletal association of the chicken AE1-4 anion exchanger in MDCK cells .
	manualset3
158276	3	411405	7	NULL	NULL	0	NULL	basolateral sorting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	AE1/F ( c ) receptor chimeras have been used to define the sequences that direct the basolateral sorting , recycling and cytoskeletal association of the chicken AE1-4 anion exchanger in MDCK cells .
	manualset3
158277	4	411405	7	NULL	NULL	0	NULL	recycling 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	AE1/F ( c ) receptor chimeras have been used to define the sequences that direct the basolateral sorting , recycling and cytoskeletal association of the chicken AE1-4 anion exchanger in MDCK cells .
	manualset3
158278	5	411405	7	NULL	NULL	0	NULL	cytoskeletal association	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	AE1/F ( c ) receptor chimeras have been used to define the sequences that direct the basolateral sorting , recycling and cytoskeletal association of the chicken AE1-4 anion exchanger in MDCK cells .
	manualset3
158279	6	411405	7	NULL	NULL	0	NULL	chicken AE1-4 anion exchanger	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	AE1/F ( c ) receptor chimeras have been used to define the sequences that direct the basolateral sorting , recycling and cytoskeletal association of the chicken AE1-4 anion exchanger in MDCK cells .
	manualset3
158280	7	411405	7	NULL	NULL	0	NULL	MDCK cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	AE1/F ( c ) receptor chimeras have been used to define the sequences that direct the basolateral sorting , recycling and cytoskeletal association of the chicken AE1-4 anion exchanger in MDCK cells .
	manualset3
158281	1	411406	7	NULL	NULL	0	NULL	 participation percentage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The participation percentage was 89.6 .
	manualset3
158282	2	411406	7	NULL	NULL	0	NULL	 89.6	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The participation percentage was 89.6 .
	manualset3
158283	1	411407	7	NULL	NULL	0	NULL	partition function	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The partition function of such a landscape can be written in terms of a density of states , which can be computed using a variety of Monte Carlo techniques .
	manualset3
158284	2	411407	7	NULL	NULL	0	NULL	landscape	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The partition function of such a landscape can be written in terms of a density of states , which can be computed using a variety of Monte Carlo techniques .
	manualset3
158285	3	411407	7	NULL	NULL	NULL	NULL	density of states	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The partition function of such a landscape can be written in terms of a density of states , which can be computed using a variety of Monte Carlo techniques .
	manualset3
158286	4	411407	7	NULL	NULL	0	NULL	Monte Carlo techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The partition function of such a landscape can be written in terms of a density of states , which can be computed using a variety of Monte Carlo techniques .
	manualset3
158287	1	411408	7	NULL	NULL	0	NULL	partitioning of entropic components	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The partitioning of entropic and enthalpic components of binding energy was confirmed by isothermal titration calorimetry with wild-type and Delta209-222 rGST A1-1 .
	manualset3
158288	2	411408	7	NULL	NULL	0	NULL	partitioning of enthalpic components 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The partitioning of entropic and enthalpic components of binding energy was confirmed by isothermal titration calorimetry with wild-type and Delta209-222 rGST A1-1 .
	manualset3
158289	3	411408	7	NULL	NULL	0	NULL	binding energy	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The partitioning of entropic and enthalpic components of binding energy was confirmed by isothermal titration calorimetry with wild-type and Delta209-222 rGST A1-1 .
	manualset3
158290	4	411408	7	NULL	NULL	0	NULL	 isothermal titration calorimetry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The partitioning of entropic and enthalpic components of binding energy was confirmed by isothermal titration calorimetry with wild-type and Delta209-222 rGST A1-1 .
	manualset3
158291	5	411408	7	NULL	NULL	0	NULL	wild-type rGST A1-1	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The partitioning of entropic and enthalpic components of binding energy was confirmed by isothermal titration calorimetry with wild-type and Delta209-222 rGST A1-1 .
	manualset3
158292	6	411408	7	NULL	NULL	0	NULL	Delta209-222 rGST A1-1	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The partitioning of entropic and enthalpic components of binding energy was confirmed by isothermal titration calorimetry with wild-type and Delta209-222 rGST A1-1 .
	manualset3
158293	1	411409	7	NULL	NULL	0	NULL	parts of the body	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The parts of the body most commonly affected were the limbs , head and neck , and central nervous system .
	manualset3
158294	2	411409	7	NULL	NULL	0	NULL	limbs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The parts of the body most commonly affected were the limbs , head and neck , and central nervous system .
	manualset3
158295	3	411409	7	NULL	NULL	0	NULL	head and neck	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The parts of the body most commonly affected were the limbs , head and neck , and central nervous system .
	manualset3
158296	4	411409	7	NULL	NULL	0	NULL	 central nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The parts of the body most commonly affected were the limbs , head and neck , and central nervous system .
	manualset3
158297	1	411410	7	NULL	NULL	NULL	NULL	past	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The past , present and future for dental hygienists .
	manualset3
158298	2	411410	7	NULL	NULL	0	NULL	present	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The past , present and future for dental hygienists .
	manualset3
158299	3	411410	7	NULL	NULL	0	NULL	future	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The past , present and future for dental hygienists .
	manualset3
158300	4	411410	7	NULL	NULL	0	NULL	dental hygienists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The past , present and future for dental hygienists .
	manualset3
158301	1	411411	7	NULL	NULL	0	NULL	patency rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The patency rate of these grafts at 6 weeks was 25 % .
	manualset3
158302	2	411411	7	NULL	NULL	0	NULL	grafts	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patency rate of these grafts at 6 weeks was 25 % .
	manualset3
158303	3	411411	7	NULL	NULL	0	NULL	6 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The patency rate of these grafts at 6 weeks was 25 % .
	manualset3
158304	4	411411	7	NULL	NULL	0	NULL	25 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The patency rate of these grafts at 6 weeks was 25 % .
	manualset3
158305	1	411412	7	NULL	NULL	0	NULL	path of determination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The path of determination : exploring the lived experience of breastfeeding difficulties .
	manualset3
158306	2	411412	7	NULL	NULL	0	NULL	experience	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The path of determination : exploring the lived experience of breastfeeding difficulties .
	manualset3
158307	3	411412	7	NULL	NULL	0	NULL	breastfeeding difficulties	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The path of determination : exploring the lived experience of breastfeeding difficulties .
	manualset3
158308	1	411413	7	NULL	NULL	NULL	NULL	pathogen-induced plant defense signaling network	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The pathogen-induced plant defense signaling network consists of multiple components , although only some of them are characterized .
	manualset3
158309	2	411413	7	NULL	NULL	NULL	NULL	multiple components	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The pathogen-induced plant defense signaling network consists of multiple components , although only some of them are characterized .
	manualset3
158310	1	411414	7	NULL	NULL	NULL	NULL	pathogenesis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The pathogenesis of hypertrophic stenosis of the pylorus in the newborn and the adult .
	manualset3
158311	2	411414	7	NULL	NULL	0	NULL	hypertrophic stenosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The pathogenesis of hypertrophic stenosis of the pylorus in the newborn and the adult .
	manualset3
158312	3	411414	7	NULL	NULL	0	NULL	pylorus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The pathogenesis of hypertrophic stenosis of the pylorus in the newborn and the adult .
	manualset3
158313	4	411414	7	NULL	NULL	0	NULL	newborn	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The pathogenesis of hypertrophic stenosis of the pylorus in the newborn and the adult .
	manualset3
158314	5	411414	7	NULL	NULL	0	NULL	 adult	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The pathogenesis of hypertrophic stenosis of the pylorus in the newborn and the adult .
	manualset3
158315	1	411415	7	NULL	NULL	0	NULL	AE3 variation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	AE3 variation may prove useful for further genetic studies , such as finer resolution mapping .
	manualset3
158316	2	411415	7	NULL	NULL	0	NULL	genetic studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	AE3 variation may prove useful for further genetic studies , such as finer resolution mapping .
	manualset3
158317	3	411415	7	NULL	NULL	0	NULL	finer resolution mapping	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	AE3 variation may prove useful for further genetic studies , such as finer resolution mapping .
	manualset3
158318	1	411416	7	NULL	NULL	0	NULL	pathogenetic mechanism 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The pathogenetic mechanism may involve cryoglobulins themselves as immune complexes ; it is also possible that monoclonal cryoglobulins combine with an antigen to form immune complexes or lead to in situ formation of immune complexes .
	manualset3
158319	2	411416	7	NULL	NULL	0	NULL	cryoglobulins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The pathogenetic mechanism may involve cryoglobulins themselves as immune complexes ; it is also possible that monoclonal cryoglobulins combine with an antigen to form immune complexes or lead to in situ formation of immune complexes .
	manualset3
158320	3	411416	7	NULL	NULL	NULL	NULL	immune complexes	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The pathogenetic mechanism may involve cryoglobulins themselves as immune complexes ; it is also possible that monoclonal cryoglobulins combine with an antigen to form immune complexes or lead to in situ formation of immune complexes .
	manualset3
158321	4	411416	7	NULL	NULL	0	NULL	monoclonal cryoglobulins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The pathogenetic mechanism may involve cryoglobulins themselves as immune complexes ; it is also possible that monoclonal cryoglobulins combine with an antigen to form immune complexes or lead to in situ formation of immune complexes .
	manualset3
158322	5	411416	7	NULL	NULL	0	NULL	antigen 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The pathogenetic mechanism may involve cryoglobulins themselves as immune complexes ; it is also possible that monoclonal cryoglobulins combine with an antigen to form immune complexes or lead to in situ formation of immune complexes .
	manualset3
158323	6	411416	7	NULL	NULL	0	NULL	immune complexes	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The pathogenetic mechanism may involve cryoglobulins themselves as immune complexes ; it is also possible that monoclonal cryoglobulins combine with an antigen to form immune complexes or lead to in situ formation of immune complexes .
	manualset3
158324	7	411416	7	NULL	NULL	0	NULL	 in situ formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The pathogenetic mechanism may involve cryoglobulins themselves as immune complexes ; it is also possible that monoclonal cryoglobulins combine with an antigen to form immune complexes or lead to in situ formation of immune complexes .
	manualset3
158325	8	411416	7	NULL	NULL	0	NULL	immune complexes	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The pathogenetic mechanism may involve cryoglobulins themselves as immune complexes ; it is also possible that monoclonal cryoglobulins combine with an antigen to form immune complexes or lead to in situ formation of immune complexes .
	manualset3
158326	1	411417	7	NULL	NULL	0	NULL	pathogenic significance of progesterone 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The pathogenic significance of progesterone in pyometra in bitches was investigated by evaluating the stages of the oestrous cycles of 369 bitches with pyometra .
	manualset3
158327	2	411417	7	NULL	NULL	0	NULL	pyometra	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The pathogenic significance of progesterone in pyometra in bitches was investigated by evaluating the stages of the oestrous cycles of 369 bitches with pyometra .
	manualset3
158328	3	411417	7	NULL	NULL	0	NULL	bitches 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The pathogenic significance of progesterone in pyometra in bitches was investigated by evaluating the stages of the oestrous cycles of 369 bitches with pyometra .
	manualset3
158329	4	411417	7	NULL	NULL	0	NULL	stages of the oestrous cycles	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The pathogenic significance of progesterone in pyometra in bitches was investigated by evaluating the stages of the oestrous cycles of 369 bitches with pyometra .
	manualset3
158330	5	411417	7	NULL	NULL	0	NULL	369 bitches	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The pathogenic significance of progesterone in pyometra in bitches was investigated by evaluating the stages of the oestrous cycles of 369 bitches with pyometra .
	manualset3
158331	6	411417	7	NULL	NULL	0	NULL	 pyometra	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The pathogenic significance of progesterone in pyometra in bitches was investigated by evaluating the stages of the oestrous cycles of 369 bitches with pyometra .
	manualset3
158332	1	411418	7	NULL	NULL	0	NULL	pathologic anatomy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The pathologic anatomy of Ebstein 's disease .
	manualset3
158333	2	411418	7	NULL	NULL	0	NULL	Ebstein 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The pathologic anatomy of Ebstein 's disease .
	manualset3
158334	1	411419	7	NULL	NULL	0	NULL	pathophysiology 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The pathophysiology of ovarian hyperstimulation syndrome ( OHSS ) remains unclear .
	manualset3
158335	2	411419	7	NULL	NULL	0	NULL	ovarian hyperstimulation syndrome ( OHSS ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The pathophysiology of ovarian hyperstimulation syndrome ( OHSS ) remains unclear .
	manualset3
158336	1	411420	7	NULL	NULL	0	NULL	patient 's ascites	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient 's ascites cleared and he remains well 10 months after surgery .
	manualset3
158337	2	411420	7	NULL	NULL	0	NULL	10 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient 's ascites cleared and he remains well 10 months after surgery .
	manualset3
158338	3	411420	7	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient 's ascites cleared and he remains well 10 months after surgery .
	manualset3
158339	1	411421	7	NULL	NULL	0	NULL	patient 's hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient 's hypertension , which had been well-controlled by long-acting nifedipine , deteriorated after the administration of rifampicin , an antitubercular agent .
	manualset3
158340	2	411421	7	NULL	NULL	0	NULL	long-acting nifedipine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient 's hypertension , which had been well-controlled by long-acting nifedipine , deteriorated after the administration of rifampicin , an antitubercular agent .
	manualset3
158341	3	411421	7	NULL	NULL	0	NULL	administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient 's hypertension , which had been well-controlled by long-acting nifedipine , deteriorated after the administration of rifampicin , an antitubercular agent .
	manualset3
158342	4	411421	7	NULL	NULL	0	NULL	rifampicin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient 's hypertension , which had been well-controlled by long-acting nifedipine , deteriorated after the administration of rifampicin , an antitubercular agent .
	manualset3
158343	5	411421	7	NULL	NULL	0	NULL	antitubercular agent	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient 's hypertension , which had been well-controlled by long-acting nifedipine , deteriorated after the administration of rifampicin , an antitubercular agent .
	manualset3
158344	1	411422	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient , a 29-year-old female , was admitted to the hospital in the 36th week of her 10th pregnancy .
	manualset3
158345	2	411422	7	NULL	NULL	0	NULL	29-year-old female	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient , a 29-year-old female , was admitted to the hospital in the 36th week of her 10th pregnancy .
	manualset3
158346	3	411422	7	NULL	NULL	0	NULL	hospital	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient , a 29-year-old female , was admitted to the hospital in the 36th week of her 10th pregnancy .
	manualset3
158347	4	411422	7	NULL	NULL	0	NULL	36th week 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient , a 29-year-old female , was admitted to the hospital in the 36th week of her 10th pregnancy .
	manualset3
158348	5	411422	7	NULL	NULL	0	NULL	10th pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient , a 29-year-old female , was admitted to the hospital in the 36th week of her 10th pregnancy .
	manualset3
158349	1	411423	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient acts as her own control in that the unoperated side shows normal suppression of otoacoustic emission amplitude with contralateral acoustic stimulation .
	manualset3
158350	2	411423	7	NULL	NULL	0	NULL	control 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient acts as her own control in that the unoperated side shows normal suppression of otoacoustic emission amplitude with contralateral acoustic stimulation .
	manualset3
158352	3	411423	7	NULL	NULL	NULL	NULL	unoperated side	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The patient acts as her own control in that the unoperated side shows normal suppression of otoacoustic emission amplitude with contralateral acoustic stimulation .
	manualset3
158353	4	411423	7	NULL	NULL	0	NULL	normal suppression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient acts as her own control in that the unoperated side shows normal suppression of otoacoustic emission amplitude with contralateral acoustic stimulation .
	manualset3
158354	5	411423	7	NULL	NULL	NULL	NULL	otoacoustic emission amplitude with contralateral acoustic stimulation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The patient acts as her own control in that the unoperated side shows normal suppression of otoacoustic emission amplitude with contralateral acoustic stimulation .
	manualset3
158355	1	411424	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient also tested positive for myeloperoxidase-antineutrophil cytoplasmic antibodies ( MPO-ANCA ) , with changes in the MPO-ANCA titer that paralleled changes in the symptoms .
	manualset3
158357	3	411424	7	NULL	NULL	0	NULL	myeloperoxidase-antineutrophil cytoplasmic antibodies ( MPO-ANCA )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient also tested positive for myeloperoxidase-antineutrophil cytoplasmic antibodies ( MPO-ANCA ) , with changes in the MPO-ANCA titer that paralleled changes in the symptoms .
	manualset3
158358	4	411424	7	NULL	NULL	NULL	NULL	MPO-ANCA titer	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The patient also tested positive for myeloperoxidase-antineutrophil cytoplasmic antibodies ( MPO-ANCA ) , with changes in the MPO-ANCA titer that paralleled changes in the symptoms .
	manualset3
158359	5	411424	7	NULL	NULL	0	NULL	symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient also tested positive for myeloperoxidase-antineutrophil cytoplasmic antibodies ( MPO-ANCA ) , with changes in the MPO-ANCA titer that paralleled changes in the symptoms .
	manualset3
158360	1	411425	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient came to the hospital with the chief complaint regarding passage dysphagia in the time of deglutition ; pharyngitis and esophageal candidiasis were found by endoscopy of upper gastrointestinal tract .
	manualset3
158361	2	411425	7	NULL	NULL	0	NULL	hospital	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient came to the hospital with the chief complaint regarding passage dysphagia in the time of deglutition ; pharyngitis and esophageal candidiasis were found by endoscopy of upper gastrointestinal tract .
	manualset3
158362	3	411425	7	NULL	NULL	0	NULL	chief complaint 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient came to the hospital with the chief complaint regarding passage dysphagia in the time of deglutition ; pharyngitis and esophageal candidiasis were found by endoscopy of upper gastrointestinal tract .
	manualset3
158363	4	411425	7	NULL	NULL	0	NULL	 passage dysphagia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient came to the hospital with the chief complaint regarding passage dysphagia in the time of deglutition ; pharyngitis and esophageal candidiasis were found by endoscopy of upper gastrointestinal tract .
	manualset3
158364	5	411425	7	NULL	NULL	0	NULL	deglutition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient came to the hospital with the chief complaint regarding passage dysphagia in the time of deglutition ; pharyngitis and esophageal candidiasis were found by endoscopy of upper gastrointestinal tract .
	manualset3
158365	6	411425	7	NULL	NULL	0	NULL	pharyngitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient came to the hospital with the chief complaint regarding passage dysphagia in the time of deglutition ; pharyngitis and esophageal candidiasis were found by endoscopy of upper gastrointestinal tract .
	manualset3
158366	7	411425	7	NULL	NULL	0	NULL	esophageal candidiasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient came to the hospital with the chief complaint regarding passage dysphagia in the time of deglutition ; pharyngitis and esophageal candidiasis were found by endoscopy of upper gastrointestinal tract .
	manualset3
158367	8	411425	7	NULL	NULL	0	NULL	endoscopy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient came to the hospital with the chief complaint regarding passage dysphagia in the time of deglutition ; pharyngitis and esophageal candidiasis were found by endoscopy of upper gastrointestinal tract .
	manualset3
158368	9	411425	7	NULL	NULL	0	NULL	upper gastrointestinal tract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient came to the hospital with the chief complaint regarding passage dysphagia in the time of deglutition ; pharyngitis and esophageal candidiasis were found by endoscopy of upper gastrointestinal tract .
	manualset3
158369	1	411426	7	NULL	NULL	0	NULL	 patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient carrying the allele 364C had a more severe hemorrhagic diathesis than the S363I mutant .
	manualset3
158370	2	411426	7	NULL	NULL	0	NULL	allele 364C	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient carrying the allele 364C had a more severe hemorrhagic diathesis than the S363I mutant .
	manualset3
158371	3	411426	7	NULL	NULL	0	NULL	severe hemorrhagic diathesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient carrying the allele 364C had a more severe hemorrhagic diathesis than the S363I mutant .
	manualset3
158372	4	411426	7	NULL	NULL	0	NULL	S363I mutant 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient carrying the allele 364C had a more severe hemorrhagic diathesis than the S363I mutant .
	manualset3
158373	1	411427	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient developed chronic nonhealing ulcers secondary to hydrocephalus , ventriculoperitoneal shunts , and the underlying architecture of her cranial vault .
	manualset3
158374	2	411427	7	NULL	NULL	0	NULL	chronic nonhealing ulcers 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient developed chronic nonhealing ulcers secondary to hydrocephalus , ventriculoperitoneal shunts , and the underlying architecture of her cranial vault .
	manualset3
158376	4	411427	7	NULL	NULL	0	NULL	hydrocephalus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient developed chronic nonhealing ulcers secondary to hydrocephalus , ventriculoperitoneal shunts , and the underlying architecture of her cranial vault .
	manualset3
158377	5	411427	7	NULL	NULL	0	NULL	ventriculoperitoneal shunts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient developed chronic nonhealing ulcers secondary to hydrocephalus , ventriculoperitoneal shunts , and the underlying architecture of her cranial vault .
	manualset3
158378	6	411427	7	NULL	NULL	0	NULL	cranial vault	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient developed chronic nonhealing ulcers secondary to hydrocephalus , ventriculoperitoneal shunts , and the underlying architecture of her cranial vault .
	manualset3
161007	7	411427	7	NULL	NULL	0	NULL	architecture 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient developed chronic nonhealing ulcers secondary to hydrocephalus , ventriculoperitoneal shunts , and the underlying architecture of her cranial vault .
	manualset3
158379	1	411428	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient had a good response to antacids and H2-blockers and remains asymptomatic after 2 years with the same treatment .
	manualset3
158380	2	411428	7	NULL	NULL	NULL	NULL	good response	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The patient had a good response to antacids and H2-blockers and remains asymptomatic after 2 years with the same treatment .
	manualset3
158381	3	411428	7	NULL	NULL	0	NULL	 antacids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient had a good response to antacids and H2-blockers and remains asymptomatic after 2 years with the same treatment .
	manualset3
158382	4	411428	7	NULL	NULL	0	NULL	H2-blockers 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient had a good response to antacids and H2-blockers and remains asymptomatic after 2 years with the same treatment .
	manualset3
158383	5	411428	7	NULL	NULL	0	NULL	2 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient had a good response to antacids and H2-blockers and remains asymptomatic after 2 years with the same treatment .
	manualset3
158384	6	411428	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient had a good response to antacids and H2-blockers and remains asymptomatic after 2 years with the same treatment .
	manualset3
158385	1	411429	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient had an uneventful post operative recovery and no recurrence in 6 months of follow up .
	manualset3
158386	2	411429	7	NULL	NULL	0	NULL	uneventful post operative recovery 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient had an uneventful post operative recovery and no recurrence in 6 months of follow up .
	manualset3
158387	3	411429	7	NULL	NULL	0	NULL	6 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient had an uneventful post operative recovery and no recurrence in 6 months of follow up .
	manualset3
158388	4	411429	7	NULL	NULL	0	NULL	follow up	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient had an uneventful post operative recovery and no recurrence in 6 months of follow up .
	manualset3
158389	1	411430	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient had been taking finasteride over the past 3 months for androgenetic alopecia .
	manualset3
158390	2	411430	7	NULL	NULL	0	NULL	finasteride	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient had been taking finasteride over the past 3 months for androgenetic alopecia .
	manualset3
158391	3	411430	7	NULL	NULL	0	NULL	3 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient had been taking finasteride over the past 3 months for androgenetic alopecia .
	manualset3
158392	4	411430	7	NULL	NULL	0	NULL	androgenetic alopecia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient had been taking finasteride over the past 3 months for androgenetic alopecia .
	manualset3
158393	1	411431	7	NULL	NULL	NULL	NULL	AET	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	AET did not alter the response to CaCl ( 2 ) in vessels exposed to KCl depolarization .
	manualset3
158394	2	411431	7	NULL	NULL	NULL	NULL	response	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	AET did not alter the response to CaCl ( 2 ) in vessels exposed to KCl depolarization .
	manualset3
158395	3	411431	7	NULL	NULL	0	NULL	CaCl ( 2 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	AET did not alter the response to CaCl ( 2 ) in vessels exposed to KCl depolarization .
	manualset3
158396	4	411431	7	NULL	NULL	NULL	NULL	vessels 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	AET did not alter the response to CaCl ( 2 ) in vessels exposed to KCl depolarization .
	manualset3
158397	5	411431	7	NULL	NULL	0	NULL	KCl depolarization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	AET did not alter the response to CaCl ( 2 ) in vessels exposed to KCl depolarization .
	manualset3
158401	1	411432	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient has been free of hiccups and has been neurologically intact since the day after total removal of the tumor .
	manualset3
158402	2	411432	7	NULL	NULL	0	NULL	hiccups	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient has been free of hiccups and has been neurologically intact since the day after total removal of the tumor .
	manualset3
158403	3	411432	7	NULL	NULL	0	NULL	day	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient has been free of hiccups and has been neurologically intact since the day after total removal of the tumor .
	manualset3
158404	4	411432	7	NULL	NULL	0	NULL	total removal	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient has been free of hiccups and has been neurologically intact since the day after total removal of the tumor .
	manualset3
158405	5	411432	7	NULL	NULL	0	NULL	tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient has been free of hiccups and has been neurologically intact since the day after total removal of the tumor .
	manualset3
158406	1	411433	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient has lived for more than 5 years after treatment on the AML99-Down protocol in Japan .
	manualset3
158407	2	411433	7	NULL	NULL	0	NULL	5 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient has lived for more than 5 years after treatment on the AML99-Down protocol in Japan .
	manualset3
158408	3	411433	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient has lived for more than 5 years after treatment on the AML99-Down protocol in Japan .
	manualset3
158409	4	411433	7	NULL	NULL	0	NULL	AML99-Down protocol	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient has lived for more than 5 years after treatment on the AML99-Down protocol in Japan .
	manualset3
158410	5	411433	7	NULL	NULL	0	NULL	Japan 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient has lived for more than 5 years after treatment on the AML99-Down protocol in Japan .
	manualset3
158411	1	411434	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient may be the 5th reported case of TA complicated with arteritis-induced intestinal perforation .
	manualset3
158412	2	411434	7	NULL	NULL	0	NULL	 5th reported case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient may be the 5th reported case of TA complicated with arteritis-induced intestinal perforation .
	manualset3
158413	3	411434	7	NULL	NULL	0	NULL	TA 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient may be the 5th reported case of TA complicated with arteritis-induced intestinal perforation .
	manualset3
158414	4	411434	7	NULL	NULL	0	NULL	arteritis-induced intestinal perforation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient may be the 5th reported case of TA complicated with arteritis-induced intestinal perforation .
	manualset3
158415	1	411435	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient met all 6 of the Centers for Disease Control and Prevention diagnostic criteria for toxic shock syndrome , and her intrauterine device grew out Staphylococcus aureus .
	manualset3
158416	2	411435	7	NULL	NULL	0	NULL	6 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient met all 6 of the Centers for Disease Control and Prevention diagnostic criteria for toxic shock syndrome , and her intrauterine device grew out Staphylococcus aureus .
	manualset3
158417	3	411435	7	NULL	NULL	0	NULL	 Centers for Disease Control and Prevention diagnostic criteria	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient met all 6 of the Centers for Disease Control and Prevention diagnostic criteria for toxic shock syndrome , and her intrauterine device grew out Staphylococcus aureus .
	manualset3
158418	4	411435	7	NULL	NULL	0	NULL	toxic shock syndrome 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient met all 6 of the Centers for Disease Control and Prevention diagnostic criteria for toxic shock syndrome , and her intrauterine device grew out Staphylococcus aureus .
	manualset3
158419	5	411435	7	NULL	NULL	0	NULL	intrauterine device	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient met all 6 of the Centers for Disease Control and Prevention diagnostic criteria for toxic shock syndrome , and her intrauterine device grew out Staphylococcus aureus .
	manualset3
158420	6	411435	7	NULL	NULL	0	NULL	Staphylococcus aureus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient met all 6 of the Centers for Disease Control and Prevention diagnostic criteria for toxic shock syndrome , and her intrauterine device grew out Staphylococcus aureus .
	manualset3
158421	1	411436	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient prefers to remain anonymous ; therefore , I am listed here as the contact person to whom queries to the author can be referred .
	manualset3
158422	2	411436	7	NULL	NULL	0	NULL	 contact person	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient prefers to remain anonymous ; therefore , I am listed here as the contact person to whom queries to the author can be referred .
	manualset3
158423	3	411436	7	NULL	NULL	0	NULL	author	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient prefers to remain anonymous ; therefore , I am listed here as the contact person to whom queries to the author can be referred .
	manualset3
158424	1	411437	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient presented a cardiorespiratory arrest during anesthesia due to myocardium infarction .
	manualset3
158425	2	411437	7	NULL	NULL	0	NULL	cardiorespiratory arrest	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient presented a cardiorespiratory arrest during anesthesia due to myocardium infarction .
	manualset3
158426	3	411437	7	NULL	NULL	0	NULL	anesthesia	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient presented a cardiorespiratory arrest during anesthesia due to myocardium infarction .
	manualset3
158427	4	411437	7	NULL	NULL	0	NULL	 myocardium infarction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient presented a cardiorespiratory arrest during anesthesia due to myocardium infarction .
	manualset3
158428	1	411438	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient presented with a dark hypopyon and markedly elevated intraocular pressure , and the diagnosis was established by culture and histopathologic examination of ocular fluid .
	manualset3
158429	2	411438	7	NULL	NULL	0	NULL	dark hypopyon 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient presented with a dark hypopyon and markedly elevated intraocular pressure , and the diagnosis was established by culture and histopathologic examination of ocular fluid .
	manualset3
158430	3	411438	7	NULL	NULL	0	NULL	elevated intraocular pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient presented with a dark hypopyon and markedly elevated intraocular pressure , and the diagnosis was established by culture and histopathologic examination of ocular fluid .
	manualset3
158431	4	411438	7	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient presented with a dark hypopyon and markedly elevated intraocular pressure , and the diagnosis was established by culture and histopathologic examination of ocular fluid .
	manualset3
158432	5	411438	7	NULL	NULL	0	NULL	culture	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient presented with a dark hypopyon and markedly elevated intraocular pressure , and the diagnosis was established by culture and histopathologic examination of ocular fluid .
	manualset3
158433	6	411438	7	NULL	NULL	0	NULL	histopathologic examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient presented with a dark hypopyon and markedly elevated intraocular pressure , and the diagnosis was established by culture and histopathologic examination of ocular fluid .
	manualset3
158434	7	411438	7	NULL	NULL	0	NULL	 ocular fluid	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient presented with a dark hypopyon and markedly elevated intraocular pressure , and the diagnosis was established by culture and histopathologic examination of ocular fluid .
	manualset3
158435	1	411439	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient received high-dose chemotherapy with peripheral blood stem cell transplantation and achieved complete remission .
	manualset3
158436	2	411439	7	NULL	NULL	0	NULL	high-dose chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient received high-dose chemotherapy with peripheral blood stem cell transplantation and achieved complete remission .
	manualset3
158437	3	411439	7	NULL	NULL	0	NULL	peripheral blood stem cell transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient received high-dose chemotherapy with peripheral blood stem cell transplantation and achieved complete remission .
	manualset3
158438	4	411439	7	NULL	NULL	0	NULL	complete remission	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient received high-dose chemotherapy with peripheral blood stem cell transplantation and achieved complete remission .
	manualset3
158439	1	411440	7	NULL	NULL	0	NULL	AF150 ( S )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	AF150 ( S ) and AF267B : M1 muscarinic agonists as innovative therapies for Alzheimer 's disease .
	manualset3
158440	2	411440	7	NULL	NULL	0	NULL	AF267B	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	AF150 ( S ) and AF267B : M1 muscarinic agonists as innovative therapies for Alzheimer 's disease .
	manualset3
158441	3	411440	7	NULL	NULL	0	NULL	M1 muscarinic agonists	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	AF150 ( S ) and AF267B : M1 muscarinic agonists as innovative therapies for Alzheimer 's disease .
	manualset3
158442	4	411440	7	NULL	NULL	0	NULL	innovative therapies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	AF150 ( S ) and AF267B : M1 muscarinic agonists as innovative therapies for Alzheimer 's disease .
	manualset3
158443	5	411440	7	NULL	NULL	0	NULL	Alzheimer 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	AF150 ( S ) and AF267B : M1 muscarinic agonists as innovative therapies for Alzheimer 's disease .
	manualset3
158444	1	411441	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient showed clinical complete remission .
	manualset3
158445	2	411441	7	NULL	NULL	0	NULL	clinical complete remission	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient showed clinical complete remission .
	manualset3
158446	1	411442	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient started receiving chemotherapy , but the scrotum metastasis grew rapidly and erupted .
	manualset3
158447	2	411442	7	NULL	NULL	0	NULL	chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient started receiving chemotherapy , but the scrotum metastasis grew rapidly and erupted .
	manualset3
158448	3	411442	7	NULL	NULL	0	NULL	scrotum metastasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient started receiving chemotherapy , but the scrotum metastasis grew rapidly and erupted .
	manualset3
158449	1	411443	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient stated that she has reproducible episodes of dizziness and near fainting when she climbs a flight of stairs and activity is limited to a slow gait .
	manualset3
158450	2	411443	7	NULL	NULL	NULL	NULL	reproducible episodes 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The patient stated that she has reproducible episodes of dizziness and near fainting when she climbs a flight of stairs and activity is limited to a slow gait .
	manualset3
158451	3	411443	7	NULL	NULL	NULL	NULL	 fainting	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The patient stated that she has reproducible episodes of dizziness and near fainting when she climbs a flight of stairs and activity is limited to a slow gait .
	manualset3
158452	4	411443	7	NULL	NULL	0	NULL	flight of stairs	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient stated that she has reproducible episodes of dizziness and near fainting when she climbs a flight of stairs and activity is limited to a slow gait .
	manualset3
158453	6	411443	7	NULL	NULL	NULL	NULL	slow gait	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The patient stated that she has reproducible episodes of dizziness and near fainting when she climbs a flight of stairs and activity is limited to a slow gait .
	manualset3
159399	5	411443	7	NULL	NULL	NULL	NULL	activity	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The patient stated that she has reproducible episodes of dizziness and near fainting when she climbs a flight of stairs and activity is limited to a slow gait .
	manualset3
159400	7	411443	7	NULL	NULL	0	NULL	dizziness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient stated that she has reproducible episodes of dizziness and near fainting when she climbs a flight of stairs and activity is limited to a slow gait .
	manualset3
158454	1	411444	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient underwent neck exploration with the finding and removal of a lipoadenoma , a rare parathyroid tumor , followed by complete and permanent remission of the disease .
	manualset3
158455	2	411444	7	NULL	NULL	0	NULL	neck exploration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient underwent neck exploration with the finding and removal of a lipoadenoma , a rare parathyroid tumor , followed by complete and permanent remission of the disease .
	manualset3
158456	3	411444	7	NULL	NULL	NULL	NULL	removal of a lipoadenoma	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The patient underwent neck exploration with the finding and removal of a lipoadenoma , a rare parathyroid tumor , followed by complete and permanent remission of the disease .
	manualset3
158457	4	411444	7	NULL	NULL	NULL	NULL	parathyroid tumor	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The patient underwent neck exploration with the finding and removal of a lipoadenoma , a rare parathyroid tumor , followed by complete and permanent remission of the disease .
	manualset3
158458	5	411444	7	NULL	NULL	0	NULL	complete and permanent remission	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient underwent neck exploration with the finding and removal of a lipoadenoma , a rare parathyroid tumor , followed by complete and permanent remission of the disease .
	manualset3
158459	6	411444	7	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient underwent neck exploration with the finding and removal of a lipoadenoma , a rare parathyroid tumor , followed by complete and permanent remission of the disease .
	manualset3
159401	7	411444	7	NULL	NULL	0	NULL	finding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient underwent neck exploration with the finding and removal of a lipoadenoma , a rare parathyroid tumor , followed by complete and permanent remission of the disease .
	manualset3
158460	1	411445	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient was 23 months old with a painless swelling of the right scrotal contents .
	manualset3
158461	2	411445	7	NULL	NULL	0	NULL	23 months old	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient was 23 months old with a painless swelling of the right scrotal contents .
	manualset3
158462	3	411445	7	NULL	NULL	0	NULL	painless swelling	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient was 23 months old with a painless swelling of the right scrotal contents .
	manualset3
158463	4	411445	7	NULL	NULL	0	NULL	right scrotal contents	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient was 23 months old with a painless swelling of the right scrotal contents .
	manualset3
158464	1	411446	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient was admitted to the hospital several times throughout her pregnancy for congestive heart failure , pulmonary edema , and headaches .
	manualset3
158465	2	411446	7	NULL	NULL	0	NULL	hospital	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient was admitted to the hospital several times throughout her pregnancy for congestive heart failure , pulmonary edema , and headaches .
	manualset3
158466	3	411446	7	NULL	NULL	0	NULL	several times	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient was admitted to the hospital several times throughout her pregnancy for congestive heart failure , pulmonary edema , and headaches .
	manualset3
158467	4	411446	7	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient was admitted to the hospital several times throughout her pregnancy for congestive heart failure , pulmonary edema , and headaches .
	manualset3
158468	5	411446	7	NULL	NULL	NULL	NULL	congestive heart failure 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The patient was admitted to the hospital several times throughout her pregnancy for congestive heart failure , pulmonary edema , and headaches .
	manualset3
158469	6	411446	7	NULL	NULL	0	NULL	pulmonary edema 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient was admitted to the hospital several times throughout her pregnancy for congestive heart failure , pulmonary edema , and headaches .
	manualset3
158470	7	411446	7	NULL	NULL	0	NULL	headaches	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient was admitted to the hospital several times throughout her pregnancy for congestive heart failure , pulmonary edema , and headaches .
	manualset3
158471	1	411447	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient was given nucleoside analogs .
	manualset3
158472	2	411447	7	NULL	NULL	0	NULL	nucleoside analogs	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient was given nucleoside analogs .
	manualset3
158473	1	411448	7	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients ( 1046 subjects , aged 28 to 89 ) were shared between 2 groups ; they received an identical premedication by midazolam , peroral administration , 3.75 mg in 1 h before surgery .
	manualset3
158474	2	411448	7	NULL	NULL	0	NULL	1046 subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients ( 1046 subjects , aged 28 to 89 ) were shared between 2 groups ; they received an identical premedication by midazolam , peroral administration , 3.75 mg in 1 h before surgery .
	manualset3
158475	3	411448	7	NULL	NULL	0	NULL	aged 28 to 89	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients ( 1046 subjects , aged 28 to 89 ) were shared between 2 groups ; they received an identical premedication by midazolam , peroral administration , 3.75 mg in 1 h before surgery .
	manualset3
158476	4	411448	7	NULL	NULL	0	NULL	2 groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients ( 1046 subjects , aged 28 to 89 ) were shared between 2 groups ; they received an identical premedication by midazolam , peroral administration , 3.75 mg in 1 h before surgery .
	manualset3
158477	5	411448	7	NULL	NULL	0	NULL	premedication	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients ( 1046 subjects , aged 28 to 89 ) were shared between 2 groups ; they received an identical premedication by midazolam , peroral administration , 3.75 mg in 1 h before surgery .
	manualset3
158478	6	411448	7	NULL	NULL	0	NULL	midazolam	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients ( 1046 subjects , aged 28 to 89 ) were shared between 2 groups ; they received an identical premedication by midazolam , peroral administration , 3.75 mg in 1 h before surgery .
	manualset3
158479	7	411448	7	NULL	NULL	0	NULL	peroral administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients ( 1046 subjects , aged 28 to 89 ) were shared between 2 groups ; they received an identical premedication by midazolam , peroral administration , 3.75 mg in 1 h before surgery .
	manualset3
158480	8	411448	7	NULL	NULL	0	NULL	3.75 mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients ( 1046 subjects , aged 28 to 89 ) were shared between 2 groups ; they received an identical premedication by midazolam , peroral administration , 3.75 mg in 1 h before surgery .
	manualset3
158481	9	411448	7	NULL	NULL	0	NULL	1 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients ( 1046 subjects , aged 28 to 89 ) were shared between 2 groups ; they received an identical premedication by midazolam , peroral administration , 3.75 mg in 1 h before surgery .
	manualset3
158482	10	411448	7	NULL	NULL	0	NULL	 surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients ( 1046 subjects , aged 28 to 89 ) were shared between 2 groups ; they received an identical premedication by midazolam , peroral administration , 3.75 mg in 1 h before surgery .
	manualset3
158483	1	411449	7	NULL	NULL	0	NULL	AFLP	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	AFLP clearly differentiated between C. botulinum groups I and II ; group-specific clusters showed & lt ; 10 % similarity between proteolytic and nonproteolytic C. botulinum strains .
	manualset3
158484	2	411449	7	NULL	NULL	0	NULL	C. botulinum groups I	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	AFLP clearly differentiated between C. botulinum groups I and II ; group-specific clusters showed & lt ; 10 % similarity between proteolytic and nonproteolytic C. botulinum strains .
	manualset3
158485	3	411449	7	NULL	NULL	0	NULL	C. botulinum group II	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	AFLP clearly differentiated between C. botulinum groups I and II ; group-specific clusters showed & lt ; 10 % similarity between proteolytic and nonproteolytic C. botulinum strains .
	manualset3
158486	4	411449	7	NULL	NULL	0	NULL	group-specific clusters	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	AFLP clearly differentiated between C. botulinum groups I and II ; group-specific clusters showed & lt ; 10 % similarity between proteolytic and nonproteolytic C. botulinum strains .
	manualset3
158487	5	411449	7	NULL	NULL	NULL	NULL	10 % similarity	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	AFLP clearly differentiated between C. botulinum groups I and II ; group-specific clusters showed & lt ; 10 % similarity between proteolytic and nonproteolytic C. botulinum strains .
	manualset3
158488	6	411449	7	NULL	NULL	0	NULL	proteolytic  C. botulinum strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	AFLP clearly differentiated between C. botulinum groups I and II ; group-specific clusters showed & lt ; 10 % similarity between proteolytic and nonproteolytic C. botulinum strains .
	manualset3
158489	7	411449	7	NULL	NULL	0	NULL	nonproteolytic C. botulinum strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	AFLP clearly differentiated between C. botulinum groups I and II ; group-specific clusters showed & lt ; 10 % similarity between proteolytic and nonproteolytic C. botulinum strains .
	manualset3
158490	1	411450	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients in group A received 20 ml/kg of HES ( 130/0 .4 ) , 10 mg/kg of T.A over 30 minutes followed by infusion of 1 mg/kg/hr over the next 12 hrs .
	manualset3
158491	2	411450	7	NULL	NULL	0	NULL	group A	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients in group A received 20 ml/kg of HES ( 130/0 .4 ) , 10 mg/kg of T.A over 30 minutes followed by infusion of 1 mg/kg/hr over the next 12 hrs .
	manualset3
158492	3	411450	7	NULL	NULL	0	NULL	20 ml/kg of HES ( 130/0 .4 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients in group A received 20 ml/kg of HES ( 130/0 .4 ) , 10 mg/kg of T.A over 30 minutes followed by infusion of 1 mg/kg/hr over the next 12 hrs .
	manualset3
158493	4	411450	7	NULL	NULL	0	NULL	10 mg/kg of T.A	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients in group A received 20 ml/kg of HES ( 130/0 .4 ) , 10 mg/kg of T.A over 30 minutes followed by infusion of 1 mg/kg/hr over the next 12 hrs .
	manualset3
158494	5	411450	7	NULL	NULL	0	NULL	30 minutes	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients in group A received 20 ml/kg of HES ( 130/0 .4 ) , 10 mg/kg of T.A over 30 minutes followed by infusion of 1 mg/kg/hr over the next 12 hrs .
	manualset3
158495	6	411450	7	NULL	NULL	0	NULL	infusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients in group A received 20 ml/kg of HES ( 130/0 .4 ) , 10 mg/kg of T.A over 30 minutes followed by infusion of 1 mg/kg/hr over the next 12 hrs .
	manualset3
158496	7	411450	7	NULL	NULL	0	NULL	 1 mg/kg/hr	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients in group A received 20 ml/kg of HES ( 130/0 .4 ) , 10 mg/kg of T.A over 30 minutes followed by infusion of 1 mg/kg/hr over the next 12 hrs .
	manualset3
158497	8	411450	7	NULL	NULL	0	NULL	 next 12 hrs	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients in group A received 20 ml/kg of HES ( 130/0 .4 ) , 10 mg/kg of T.A over 30 minutes followed by infusion of 1 mg/kg/hr over the next 12 hrs .
	manualset3
158498	1	411451	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients received either high-dose hemithorax irradiation for pleural mesothelioma ( 11 patients ) or high-dose irradiation with individually shaped fields for non-small cell lung cancer ( 12 patients ) .
	manualset3
158499	2	411451	7	NULL	NULL	NULL	NULL	high-dose hemithorax irradiation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The patients received either high-dose hemithorax irradiation for pleural mesothelioma ( 11 patients ) or high-dose irradiation with individually shaped fields for non-small cell lung cancer ( 12 patients ) .
	manualset3
158500	3	411451	7	NULL	NULL	0	NULL	pleural mesothelioma ( 11 patients ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients received either high-dose hemithorax irradiation for pleural mesothelioma ( 11 patients ) or high-dose irradiation with individually shaped fields for non-small cell lung cancer ( 12 patients ) .
	manualset3
158501	4	411451	7	NULL	NULL	0	NULL	high-dose irradiation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients received either high-dose hemithorax irradiation for pleural mesothelioma ( 11 patients ) or high-dose irradiation with individually shaped fields for non-small cell lung cancer ( 12 patients ) .
	manualset3
158502	5	411451	7	NULL	NULL	0	NULL	individually shaped fields	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients received either high-dose hemithorax irradiation for pleural mesothelioma ( 11 patients ) or high-dose irradiation with individually shaped fields for non-small cell lung cancer ( 12 patients ) .
	manualset3
158503	6	411451	7	NULL	NULL	0	NULL	non-small cell lung cancer ( 12 patients )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients received either high-dose hemithorax irradiation for pleural mesothelioma ( 11 patients ) or high-dose irradiation with individually shaped fields for non-small cell lung cancer ( 12 patients ) .
	manualset3
158504	1	411452	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients reported ruptured disc to be due to lifting ( 30.13 % ) , trauma ( 9.42 % ) , and sports ( 8.11 % ) .
	manualset3
158505	2	411452	7	NULL	NULL	0	NULL	ruptured disc	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients reported ruptured disc to be due to lifting ( 30.13 % ) , trauma ( 9.42 % ) , and sports ( 8.11 % ) .
	manualset3
158506	3	411452	7	NULL	NULL	0	NULL	lifting ( 30.13 % )	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients reported ruptured disc to be due to lifting ( 30.13 % ) , trauma ( 9.42 % ) , and sports ( 8.11 % ) .
	manualset3
158507	4	411452	7	NULL	NULL	0	NULL	trauma ( 9.42 % )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients reported ruptured disc to be due to lifting ( 30.13 % ) , trauma ( 9.42 % ) , and sports ( 8.11 % ) .
	manualset3
158508	5	411452	7	NULL	NULL	0	NULL	sports ( 8.11 % )	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients reported ruptured disc to be due to lifting ( 30.13 % ) , trauma ( 9.42 % ) , and sports ( 8.11 % ) .
	manualset3
158528	1	411453	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were classified into the 4 subtypes of renal hypouricemia : ( defective presecretory reabsorption ( Pre ) , defective postsecretory reabsorption ( Post ) , enhanced tubular secretion ( Secretion ) , and defective presecretory and postsecretory reabsorption ( Pre & Post ) as based on a pharmacological test .
	manualset3
158529	2	411453	7	NULL	NULL	0	NULL	4 subtypes 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were classified into the 4 subtypes of renal hypouricemia : ( defective presecretory reabsorption ( Pre ) , defective postsecretory reabsorption ( Post ) , enhanced tubular secretion ( Secretion ) , and defective presecretory and postsecretory reabsorption ( Pre & Post ) as based on a pharmacological test .
	manualset3
158530	3	411453	7	NULL	NULL	0	NULL	renal hypouricemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were classified into the 4 subtypes of renal hypouricemia : ( defective presecretory reabsorption ( Pre ) , defective postsecretory reabsorption ( Post ) , enhanced tubular secretion ( Secretion ) , and defective presecretory and postsecretory reabsorption ( Pre & Post ) as based on a pharmacological test .
	manualset3
158531	4	411453	7	NULL	NULL	0	NULL	 defective presecretory reabsorption ( Pre )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were classified into the 4 subtypes of renal hypouricemia : ( defective presecretory reabsorption ( Pre ) , defective postsecretory reabsorption ( Post ) , enhanced tubular secretion ( Secretion ) , and defective presecretory and postsecretory reabsorption ( Pre & Post ) as based on a pharmacological test .
	manualset3
158532	5	411453	7	NULL	NULL	0	NULL	defective postsecretory reabsorption ( Post ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were classified into the 4 subtypes of renal hypouricemia : ( defective presecretory reabsorption ( Pre ) , defective postsecretory reabsorption ( Post ) , enhanced tubular secretion ( Secretion ) , and defective presecretory and postsecretory reabsorption ( Pre & Post ) as based on a pharmacological test .
	manualset3
158533	6	411453	7	NULL	NULL	0	NULL	enhanced tubular secretion ( Secretion ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were classified into the 4 subtypes of renal hypouricemia : ( defective presecretory reabsorption ( Pre ) , defective postsecretory reabsorption ( Post ) , enhanced tubular secretion ( Secretion ) , and defective presecretory and postsecretory reabsorption ( Pre & Post ) as based on a pharmacological test .
	manualset3
158534	7	411453	7	NULL	NULL	0	NULL	defective presecretory and postsecretory reabsorption ( Pre & Post )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were classified into the 4 subtypes of renal hypouricemia : ( defective presecretory reabsorption ( Pre ) , defective postsecretory reabsorption ( Post ) , enhanced tubular secretion ( Secretion ) , and defective presecretory and postsecretory reabsorption ( Pre & Post ) as based on a pharmacological test .
	manualset3
158535	8	411453	7	NULL	NULL	0	NULL	pharmacological test	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were classified into the 4 subtypes of renal hypouricemia : ( defective presecretory reabsorption ( Pre ) , defective postsecretory reabsorption ( Post ) , enhanced tubular secretion ( Secretion ) , and defective presecretory and postsecretory reabsorption ( Pre & Post ) as based on a pharmacological test .
	manualset3
158536	1	411454	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were classified into two groups : distribution of intrahepatic radioactivity of 201Tl and/or 99Tcm-pertechnetate scintigrams similar to ( homogeneous ) or different from ( heterogeneous ) that of 99Tcm-Sn-colloid scintigrams .
	manualset3
158537	2	411454	7	NULL	NULL	0	NULL	two groups 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were classified into two groups : distribution of intrahepatic radioactivity of 201Tl and/or 99Tcm-pertechnetate scintigrams similar to ( homogeneous ) or different from ( heterogeneous ) that of 99Tcm-Sn-colloid scintigrams .
	manualset3
158538	3	411454	7	NULL	NULL	NULL	NULL	distribution 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The patients were classified into two groups : distribution of intrahepatic radioactivity of 201Tl and/or 99Tcm-pertechnetate scintigrams similar to ( homogeneous ) or different from ( heterogeneous ) that of 99Tcm-Sn-colloid scintigrams .
	manualset3
158539	4	411454	7	NULL	NULL	0	NULL	99Tcm-pertechnetate scintigrams	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were classified into two groups : distribution of intrahepatic radioactivity of 201Tl and/or 99Tcm-pertechnetate scintigrams similar to ( homogeneous ) or different from ( heterogeneous ) that of 99Tcm-Sn-colloid scintigrams .
	manualset3
158542	5	411454	7	NULL	NULL	NULL	NULL	99Tcm-Sn-colloid scintigrams	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The patients were classified into two groups : distribution of intrahepatic radioactivity of 201Tl and/or 99Tcm-pertechnetate scintigrams similar to ( homogeneous ) or different from ( heterogeneous ) that of 99Tcm-Sn-colloid scintigrams .
	manualset3
159402	6	411454	7	NULL	NULL	NULL	NULL	intrahepatic radioactivity of 201Tl	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The patients were classified into two groups : distribution of intrahepatic radioactivity of 201Tl and/or 99Tcm-pertechnetate scintigrams similar to ( homogeneous ) or different from ( heterogeneous ) that of 99Tcm-Sn-colloid scintigrams .
	manualset3
158543	1	411455	7	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were compared for hemodynamic changes before the start of the surgery , after induction , 1 , 3 , and 5 min after intubation .
	manualset3
158544	2	411455	7	NULL	NULL	0	NULL	hemodynamic changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were compared for hemodynamic changes before the start of the surgery , after induction , 1 , 3 , and 5 min after intubation .
	manualset3
158545	3	411455	7	NULL	NULL	NULL	NULL	 start 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The patients were compared for hemodynamic changes before the start of the surgery , after induction , 1 , 3 , and 5 min after intubation .
	manualset3
158546	4	411455	7	NULL	NULL	NULL	NULL	induction	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The patients were compared for hemodynamic changes before the start of the surgery , after induction , 1 , 3 , and 5 min after intubation .
	manualset3
158547	5	411455	7	NULL	NULL	0	NULL	1 , 3 , and 5 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were compared for hemodynamic changes before the start of the surgery , after induction , 1 , 3 , and 5 min after intubation .
	manualset3
158548	6	411455	7	NULL	NULL	NULL	NULL	intubation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The patients were compared for hemodynamic changes before the start of the surgery , after induction , 1 , 3 , and 5 min after intubation .
	manualset3
159403	7	411455	7	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were compared for hemodynamic changes before the start of the surgery , after induction , 1 , 3 , and 5 min after intubation .
	manualset3
158549	1	411456	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were examined with the pacemaker programmed in the VVI and VDD modes .
	manualset3
158550	2	411456	7	NULL	NULL	0	NULL	pacemaker	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were examined with the pacemaker programmed in the VVI and VDD modes .
	manualset3
158551	3	411456	7	NULL	NULL	0	NULL	VVI modes	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were examined with the pacemaker programmed in the VVI and VDD modes .
	manualset3
158552	4	411456	7	NULL	NULL	0	NULL	VDD modes	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were examined with the pacemaker programmed in the VVI and VDD modes .
	manualset3
158553	1	411457	7	NULL	NULL	0	NULL	AFM analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	AFM analysis exhibited relatively less aggregation of nanoparticles for microwave assisted process .
	manualset3
158554	2	411457	7	NULL	NULL	NULL	NULL	less aggregation 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	AFM analysis exhibited relatively less aggregation of nanoparticles for microwave assisted process .
	manualset3
158555	4	411457	7	NULL	NULL	NULL	NULL	microwave assisted process	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	AFM analysis exhibited relatively less aggregation of nanoparticles for microwave assisted process .
	manualset3
159404	3	411457	7	NULL	NULL	0	NULL	nanoparticles	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	AFM analysis exhibited relatively less aggregation of nanoparticles for microwave assisted process .
	manualset3
158556	1	411458	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were randomly allocated to receive either capsules of placebo or capsules of 5 mg of isradipine and were reinvestigated after 2 h and 3 months .
	manualset3
158558	3	411458	7	NULL	NULL	NULL	NULL	placebo	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The patients were randomly allocated to receive either capsules of placebo or capsules of 5 mg of isradipine and were reinvestigated after 2 h and 3 months .
	manualset3
158559	4	411458	7	NULL	NULL	NULL	NULL	capsules 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The patients were randomly allocated to receive either capsules of placebo or capsules of 5 mg of isradipine and were reinvestigated after 2 h and 3 months .
	manualset3
158560	7	411458	7	NULL	NULL	NULL	NULL	 2 h and 3 months	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The patients were randomly allocated to receive either capsules of placebo or capsules of 5 mg of isradipine and were reinvestigated after 2 h and 3 months .
	manualset3
159405	2	411458	7	NULL	NULL	0	NULL	capsules	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were randomly allocated to receive either capsules of placebo or capsules of 5 mg of isradipine and were reinvestigated after 2 h and 3 months .
	manualset3
159406	5	411458	7	NULL	NULL	0	NULL	5 mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were randomly allocated to receive either capsules of placebo or capsules of 5 mg of isradipine and were reinvestigated after 2 h and 3 months .
	manualset3
159407	6	411458	7	NULL	NULL	0	NULL	isradipine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were randomly allocated to receive either capsules of placebo or capsules of 5 mg of isradipine and were reinvestigated after 2 h and 3 months .
	manualset3
158561	1	411459	7	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were reassessed from one month to nine years after the development of the IION ( mean follow-up was 4.6 years ) .
	manualset3
158562	2	411459	7	NULL	NULL	0	NULL	one month to nine years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were reassessed from one month to nine years after the development of the IION ( mean follow-up was 4.6 years ) .
	manualset3
158563	3	411459	7	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were reassessed from one month to nine years after the development of the IION ( mean follow-up was 4.6 years ) .
	manualset3
158564	4	411459	7	NULL	NULL	0	NULL	IION	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were reassessed from one month to nine years after the development of the IION ( mean follow-up was 4.6 years ) .
	manualset3
158565	5	411459	7	NULL	NULL	NULL	NULL	mean follow-up 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The patients were reassessed from one month to nine years after the development of the IION ( mean follow-up was 4.6 years ) .
	manualset3
158566	6	411459	7	NULL	NULL	0	NULL	 4.6 years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were reassessed from one month to nine years after the development of the IION ( mean follow-up was 4.6 years ) .
	manualset3
158567	1	411460	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients with constrictive pericarditis also showed a decrease in the physiological filling asynchrony , as assessed by segmental evaluations .
	manualset3
158568	2	411460	7	NULL	NULL	0	NULL	constrictive pericarditis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients with constrictive pericarditis also showed a decrease in the physiological filling asynchrony , as assessed by segmental evaluations .
	manualset3
158569	3	411460	7	NULL	NULL	0	NULL	decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients with constrictive pericarditis also showed a decrease in the physiological filling asynchrony , as assessed by segmental evaluations .
	manualset3
158570	4	411460	7	NULL	NULL	0	NULL	physiological filling asynchrony	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients with constrictive pericarditis also showed a decrease in the physiological filling asynchrony , as assessed by segmental evaluations .
	manualset3
158571	5	411460	7	NULL	NULL	0	NULL	segmental evaluations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients with constrictive pericarditis also showed a decrease in the physiological filling asynchrony , as assessed by segmental evaluations .
	manualset3
158572	1	411461	7	NULL	NULL	0	NULL	pattern of cancer	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The pattern of cancer in stage A2 differs from that in stage A1 in that most large transition zone cancers are selected into this stage and some of these are nondiploid .
	manualset3
158573	2	411461	7	NULL	NULL	0	NULL	stage A2	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The pattern of cancer in stage A2 differs from that in stage A1 in that most large transition zone cancers are selected into this stage and some of these are nondiploid .
	manualset3
158574	3	411461	7	NULL	NULL	0	NULL	stage A1	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The pattern of cancer in stage A2 differs from that in stage A1 in that most large transition zone cancers are selected into this stage and some of these are nondiploid .
	manualset3
158575	4	411461	7	NULL	NULL	0	NULL	large transition zone cancers	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The pattern of cancer in stage A2 differs from that in stage A1 in that most large transition zone cancers are selected into this stage and some of these are nondiploid .
	manualset3
158576	5	411461	7	NULL	NULL	0	NULL	stage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The pattern of cancer in stage A2 differs from that in stage A1 in that most large transition zone cancers are selected into this stage and some of these are nondiploid .
	manualset3
158577	6	411461	7	NULL	NULL	0	NULL	nondiploid	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The pattern of cancer in stage A2 differs from that in stage A1 in that most large transition zone cancers are selected into this stage and some of these are nondiploid .
	manualset3
158578	1	411462	7	NULL	NULL	0	NULL	pattern of injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The pattern of injury was similar to that associated with some other nephrotoxic and ischaemic models of acute renal failure .
	manualset3
158579	2	411462	7	NULL	NULL	0	NULL	nephrotoxic models of acute renal failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The pattern of injury was similar to that associated with some other nephrotoxic and ischaemic models of acute renal failure .
	manualset3
158580	3	411462	7	NULL	NULL	0	NULL	ischaemic models of acute renal failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The pattern of injury was similar to that associated with some other nephrotoxic and ischaemic models of acute renal failure .
	manualset3
158581	1	411463	7	NULL	NULL	NULL	NULL	 patterned substrate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The patterned substrate is immersed in an isooctane solution containing 1H , 1H , 2H , 2H-per-fluorodecyltrichlorosilane to form hydrophobic patches on the exposed surface .
	manualset3
158582	2	411463	7	NULL	NULL	0	NULL	isooctane solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The patterned substrate is immersed in an isooctane solution containing 1H , 1H , 2H , 2H-per-fluorodecyltrichlorosilane to form hydrophobic patches on the exposed surface .
	manualset3
158583	3	411463	7	NULL	NULL	0	NULL	 1H , 1H , 2H , 2H-per-fluorodecyltrichlorosilane	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The patterned substrate is immersed in an isooctane solution containing 1H , 1H , 2H , 2H-per-fluorodecyltrichlorosilane to form hydrophobic patches on the exposed surface .
	manualset3
158584	4	411463	7	NULL	NULL	0	NULL	 hydrophobic patches	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The patterned substrate is immersed in an isooctane solution containing 1H , 1H , 2H , 2H-per-fluorodecyltrichlorosilane to form hydrophobic patches on the exposed surface .
	manualset3
158585	5	411463	7	NULL	NULL	0	NULL	exposed surface	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The patterned substrate is immersed in an isooctane solution containing 1H , 1H , 2H , 2H-per-fluorodecyltrichlorosilane to form hydrophobic patches on the exposed surface .
	manualset3
158586	1	411464	7	NULL	NULL	0	NULL	 patterns of genotoxicity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The patterns of genotoxicity of quercetin for different genetic endpoints are subject to a variety of factors ( pH , antioxidants , metabolism ) whose precise role in each test remains unclear .
	manualset3
158587	2	411464	7	NULL	NULL	0	NULL	quercetin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The patterns of genotoxicity of quercetin for different genetic endpoints are subject to a variety of factors ( pH , antioxidants , metabolism ) whose precise role in each test remains unclear .
	manualset3
158588	3	411464	7	NULL	NULL	0	NULL	genetic endpoints	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The patterns of genotoxicity of quercetin for different genetic endpoints are subject to a variety of factors ( pH , antioxidants , metabolism ) whose precise role in each test remains unclear .
	manualset3
158589	4	411464	7	NULL	NULL	0	NULL	variety of factors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The patterns of genotoxicity of quercetin for different genetic endpoints are subject to a variety of factors ( pH , antioxidants , metabolism ) whose precise role in each test remains unclear .
	manualset3
158590	5	411464	7	NULL	NULL	0	NULL	pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The patterns of genotoxicity of quercetin for different genetic endpoints are subject to a variety of factors ( pH , antioxidants , metabolism ) whose precise role in each test remains unclear .
	manualset3
158591	6	411464	7	NULL	NULL	NULL	NULL	antioxidants	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The patterns of genotoxicity of quercetin for different genetic endpoints are subject to a variety of factors ( pH , antioxidants , metabolism ) whose precise role in each test remains unclear .
	manualset3
158592	7	411464	7	NULL	NULL	NULL	NULL	metabolism	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The patterns of genotoxicity of quercetin for different genetic endpoints are subject to a variety of factors ( pH , antioxidants , metabolism ) whose precise role in each test remains unclear .
	manualset3
158593	8	411464	7	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The patterns of genotoxicity of quercetin for different genetic endpoints are subject to a variety of factors ( pH , antioxidants , metabolism ) whose precise role in each test remains unclear .
	manualset3
158594	9	411464	7	NULL	NULL	0	NULL	test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The patterns of genotoxicity of quercetin for different genetic endpoints are subject to a variety of factors ( pH , antioxidants , metabolism ) whose precise role in each test remains unclear .
	manualset3
158595	1	411465	7	NULL	NULL	0	NULL	patterns 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The patterns were then used as templates to direct the self-assembly of silica colloidal spheres , forming colloidal assemblies with well-controlled sizes , shapes , and structures .
	manualset3
158596	2	411465	7	NULL	NULL	0	NULL	 templates 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The patterns were then used as templates to direct the self-assembly of silica colloidal spheres , forming colloidal assemblies with well-controlled sizes , shapes , and structures .
	manualset3
158597	3	411465	7	NULL	NULL	0	NULL	 self-assembly	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The patterns were then used as templates to direct the self-assembly of silica colloidal spheres , forming colloidal assemblies with well-controlled sizes , shapes , and structures .
	manualset3
158598	4	411465	7	NULL	NULL	0	NULL	silica colloidal spheres	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The patterns were then used as templates to direct the self-assembly of silica colloidal spheres , forming colloidal assemblies with well-controlled sizes , shapes , and structures .
	manualset3
158599	5	411465	7	NULL	NULL	0	NULL	colloidal assemblies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The patterns were then used as templates to direct the self-assembly of silica colloidal spheres , forming colloidal assemblies with well-controlled sizes , shapes , and structures .
	manualset3
158600	6	411465	7	NULL	NULL	0	NULL	well-controlled sizes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The patterns were then used as templates to direct the self-assembly of silica colloidal spheres , forming colloidal assemblies with well-controlled sizes , shapes , and structures .
	manualset3
158601	7	411465	7	NULL	NULL	NULL	NULL	shapes	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The patterns were then used as templates to direct the self-assembly of silica colloidal spheres , forming colloidal assemblies with well-controlled sizes , shapes , and structures .
	manualset3
158602	8	411465	7	NULL	NULL	NULL	NULL	structures	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The patterns were then used as templates to direct the self-assembly of silica colloidal spheres , forming colloidal assemblies with well-controlled sizes , shapes , and structures .
	manualset3
158603	1	411466	7	NULL	NULL	0	NULL	Clinical preference	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical preference of combined renoscintiphotography and ultrasonography in the renal mass diagnoses ( author 's transl ) ) .
	manualset3
158604	2	411466	7	NULL	NULL	0	NULL	combined renoscintiphotography	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical preference of combined renoscintiphotography and ultrasonography in the renal mass diagnoses ( author 's transl ) ) .
	manualset3
158605	3	411466	7	NULL	NULL	0	NULL	ultrasonography	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical preference of combined renoscintiphotography and ultrasonography in the renal mass diagnoses ( author 's transl ) ) .
	manualset3
158606	4	411466	7	NULL	NULL	0	NULL	renal mass diagnoses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical preference of combined renoscintiphotography and ultrasonography in the renal mass diagnoses ( author 's transl ) ) .
	manualset3
158607	5	411466	7	NULL	NULL	0	NULL	author 's transl	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical preference of combined renoscintiphotography and ultrasonography in the renal mass diagnoses ( author 's transl ) ) .
	manualset3
158608	1	411467	7	NULL	NULL	0	NULL	AG1024	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	AG1024 inhibited the mitogen-activated protein kinase/extracellular signal-regulated kinase pathway and restored pRb tumor suppressive function .
	manualset3
158609	2	411467	7	NULL	NULL	NULL	NULL	mitogen-activated protein kinase pathway	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	AG1024 inhibited the mitogen-activated protein kinase/extracellular signal-regulated kinase pathway and restored pRb tumor suppressive function .
	manualset3
158610	3	411467	7	NULL	NULL	0	NULL	extracellular signal-regulated kinase pathway 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	AG1024 inhibited the mitogen-activated protein kinase/extracellular signal-regulated kinase pathway and restored pRb tumor suppressive function .
	manualset3
158611	4	411467	7	NULL	NULL	0	NULL	pRb tumor suppressive function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	AG1024 inhibited the mitogen-activated protein kinase/extracellular signal-regulated kinase pathway and restored pRb tumor suppressive function .
	manualset3
158612	2	411468	7	NULL	NULL	NULL	NULL	 symmetric axosomatic synapses 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The paucity of symmetric axosomatic synapses in the rostral division may correlate with this region 's vulnerability in certain diseases .
	manualset3
158613	3	411468	7	NULL	NULL	NULL	NULL	rostral division	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The paucity of symmetric axosomatic synapses in the rostral division may correlate with this region 's vulnerability in certain diseases .
	manualset3
158614	4	411468	7	NULL	NULL	NULL	NULL	region 's vulnerability	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The paucity of symmetric axosomatic synapses in the rostral division may correlate with this region 's vulnerability in certain diseases .
	manualset3
158615	5	411468	7	NULL	NULL	NULL	NULL	diseases	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The paucity of symmetric axosomatic synapses in the rostral division may correlate with this region 's vulnerability in certain diseases .
	manualset3
159408	1	411468	7	NULL	NULL	0	NULL	 paucity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The paucity of symmetric axosomatic synapses in the rostral division may correlate with this region 's vulnerability in certain diseases .
	manualset3
158616	1	411469	7	NULL	NULL	NULL	NULL	peak-to-peak amplitude 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The peak-to-peak amplitude of the flow glottogram pulses shows a strong relationship with the amplitude of the source spectrum fundamental and varies considerably during phonation , presumably depending on the degree of glottal ab/adduction .
	manualset3
158617	2	411469	7	NULL	NULL	0	NULL	 flow glottogram pulses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The peak-to-peak amplitude of the flow glottogram pulses shows a strong relationship with the amplitude of the source spectrum fundamental and varies considerably during phonation , presumably depending on the degree of glottal ab/adduction .
	manualset3
158618	3	411469	7	NULL	NULL	0	NULL	strong relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The peak-to-peak amplitude of the flow glottogram pulses shows a strong relationship with the amplitude of the source spectrum fundamental and varies considerably during phonation , presumably depending on the degree of glottal ab/adduction .
	manualset3
158619	4	411469	7	NULL	NULL	NULL	NULL	amplitude	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The peak-to-peak amplitude of the flow glottogram pulses shows a strong relationship with the amplitude of the source spectrum fundamental and varies considerably during phonation , presumably depending on the degree of glottal ab/adduction .
	manualset3
158620	5	411469	7	NULL	NULL	NULL	NULL	source spectrum 	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The peak-to-peak amplitude of the flow glottogram pulses shows a strong relationship with the amplitude of the source spectrum fundamental and varies considerably during phonation , presumably depending on the degree of glottal ab/adduction .
	manualset3
158621	6	411469	7	NULL	NULL	0	NULL	phonation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The peak-to-peak amplitude of the flow glottogram pulses shows a strong relationship with the amplitude of the source spectrum fundamental and varies considerably during phonation , presumably depending on the degree of glottal ab/adduction .
	manualset3
158622	8	411469	7	NULL	NULL	NULL	NULL	glottal ab/adduction	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The peak-to-peak amplitude of the flow glottogram pulses shows a strong relationship with the amplitude of the source spectrum fundamental and varies considerably during phonation , presumably depending on the degree of glottal ab/adduction .
	manualset3
159409	7	411469	7	NULL	NULL	NULL	NULL	degree	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The peak-to-peak amplitude of the flow glottogram pulses shows a strong relationship with the amplitude of the source spectrum fundamental and varies considerably during phonation , presumably depending on the degree of glottal ab/adduction .
	manualset3
158623	1	411470	7	NULL	NULL	NULL	NULL	peak period	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The peak period of incidents were during the hottest part of the summer and often associated with transferring of manure for application to crop ground .
	manualset3
158624	3	411470	7	NULL	NULL	NULL	NULL	hottest part of the summer 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The peak period of incidents were during the hottest part of the summer and often associated with transferring of manure for application to crop ground .
	manualset3
158625	4	411470	7	NULL	NULL	NULL	NULL	manure	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The peak period of incidents were during the hottest part of the summer and often associated with transferring of manure for application to crop ground .
	manualset3
158626	4	411470	7	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The peak period of incidents were during the hottest part of the summer and often associated with transferring of manure for application to crop ground .
	manualset3
158627	5	411470	7	NULL	NULL	NULL	NULL	crop ground	GeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The peak period of incidents were during the hottest part of the summer and often associated with transferring of manure for application to crop ground .
	manualset3
158652	2	411470	7	NULL	NULL	0	NULL	incidents	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The peak period of incidents were during the hottest part of the summer and often associated with transferring of manure for application to crop ground .
	manualset3
158628	1	411471	7	NULL	NULL	0	NULL	peak tension	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The peak tension and total tension ( the tension-time integral -- area -- of K + contractures ) were increased by adrenaline and isoprenaline .
	manualset3
158629	2	411471	7	NULL	NULL	0	NULL	total tension	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The peak tension and total tension ( the tension-time integral -- area -- of K + contractures ) were increased by adrenaline and isoprenaline .
	manualset3
158630	3	411471	7	NULL	NULL	0	NULL	tension-time integral -- area -- of K + contractures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The peak tension and total tension ( the tension-time integral -- area -- of K + contractures ) were increased by adrenaline and isoprenaline .
	manualset3
158631	4	411471	7	NULL	NULL	0	NULL	adrenaline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The peak tension and total tension ( the tension-time integral -- area -- of K + contractures ) were increased by adrenaline and isoprenaline .
	manualset3
158632	5	411471	7	NULL	NULL	0	NULL	isoprenaline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The peak tension and total tension ( the tension-time integral -- area -- of K + contractures ) were increased by adrenaline and isoprenaline .
	manualset3
158633	1	411472	7	NULL	NULL	0	NULL	pediatrician 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The pediatrician can provide much needed support and affirmation when the mother is sabotaged by well-meaning friends and relatives who are misinformed about the value or techniques of breast-feeding .
	manualset3
158634	2	411472	7	NULL	NULL	0	NULL	support	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The pediatrician can provide much needed support and affirmation when the mother is sabotaged by well-meaning friends and relatives who are misinformed about the value or techniques of breast-feeding .
	manualset3
158635	3	411472	7	NULL	NULL	0	NULL	affirmation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The pediatrician can provide much needed support and affirmation when the mother is sabotaged by well-meaning friends and relatives who are misinformed about the value or techniques of breast-feeding .
	manualset3
158636	4	411472	7	NULL	NULL	0	NULL	mother	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The pediatrician can provide much needed support and affirmation when the mother is sabotaged by well-meaning friends and relatives who are misinformed about the value or techniques of breast-feeding .
	manualset3
158637	5	411472	7	NULL	NULL	0	NULL	well-meaning friends	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The pediatrician can provide much needed support and affirmation when the mother is sabotaged by well-meaning friends and relatives who are misinformed about the value or techniques of breast-feeding .
	manualset3
158638	6	411472	7	NULL	NULL	NULL	NULL	 relatives	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The pediatrician can provide much needed support and affirmation when the mother is sabotaged by well-meaning friends and relatives who are misinformed about the value or techniques of breast-feeding .
	manualset3
158639	7	411472	7	NULL	NULL	NULL	NULL	value	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The pediatrician can provide much needed support and affirmation when the mother is sabotaged by well-meaning friends and relatives who are misinformed about the value or techniques of breast-feeding .
	manualset3
158640	8	411472	7	NULL	NULL	0	NULL	techniques	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The pediatrician can provide much needed support and affirmation when the mother is sabotaged by well-meaning friends and relatives who are misinformed about the value or techniques of breast-feeding .
	manualset3
158641	9	411472	7	NULL	NULL	NULL	NULL	breast-feeding	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The pediatrician can provide much needed support and affirmation when the mother is sabotaged by well-meaning friends and relatives who are misinformed about the value or techniques of breast-feeding .
	manualset3
158642	1	411473	7	NULL	NULL	NULL	NULL	penetration 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The penetration of host surfaces is accompanied by the release of penetration gland products and the shedding of highly antigenic surface components ( miracidial ciliated plates and cercarial glycocalyx ) which trigger host immune reactions .
	manualset3
158643	3	411473	7	NULL	NULL	NULL	NULL	release	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The penetration of host surfaces is accompanied by the release of penetration gland products and the shedding of highly antigenic surface components ( miracidial ciliated plates and cercarial glycocalyx ) which trigger host immune reactions .
	manualset3
158644	5	411473	7	NULL	NULL	NULL	NULL	shedding 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The penetration of host surfaces is accompanied by the release of penetration gland products and the shedding of highly antigenic surface components ( miracidial ciliated plates and cercarial glycocalyx ) which trigger host immune reactions .
	manualset3
158645	7	411473	7	NULL	NULL	NULL	NULL	miracidial ciliated plates	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The penetration of host surfaces is accompanied by the release of penetration gland products and the shedding of highly antigenic surface components ( miracidial ciliated plates and cercarial glycocalyx ) which trigger host immune reactions .
	manualset3
158646	8	411473	7	NULL	NULL	NULL	NULL	cercarial glycocalyx 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The penetration of host surfaces is accompanied by the release of penetration gland products and the shedding of highly antigenic surface components ( miracidial ciliated plates and cercarial glycocalyx ) which trigger host immune reactions .
	manualset3
158647	2	411473	7	NULL	NULL	NULL	NULL	host surfaces	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The penetration of host surfaces is accompanied by the release of penetration gland products and the shedding of highly antigenic surface components ( miracidial ciliated plates and cercarial glycocalyx ) which trigger host immune reactions .
	manualset3
158648	4	411473	7	NULL	NULL	0	NULL	penetration gland products	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The penetration of host surfaces is accompanied by the release of penetration gland products and the shedding of highly antigenic surface components ( miracidial ciliated plates and cercarial glycocalyx ) which trigger host immune reactions .
	manualset3
158649	6	411473	7	NULL	NULL	NULL	NULL	highly antigenic surface components	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The penetration of host surfaces is accompanied by the release of penetration gland products and the shedding of highly antigenic surface components ( miracidial ciliated plates and cercarial glycocalyx ) which trigger host immune reactions .
	manualset3
158651	10	411473	7	NULL	NULL	0	NULL	host immune reactions .	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The penetration of host surfaces is accompanied by the release of penetration gland products and the shedding of highly antigenic surface components ( miracidial ciliated plates and cercarial glycocalyx ) which trigger host immune reactions .
	manualset3
158653	1	411474	7	NULL	NULL	0	NULL	peptide conformation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The peptide conformation is more stable in DMPC bilayer .
	manualset3
158655	2	411474	7	NULL	NULL	NULL	NULL	DMPC bilayer	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The peptide conformation is more stable in DMPC bilayer .
	manualset3
158656	1	411475	7	NULL	NULL	0	NULL	peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The peptide is a disulphide-constrained 7-mer with the amino acid sequence CTTMHPRLC that binds to nicotinic acetylcholine receptors .
	manualset3
158657	2	411475	7	NULL	NULL	0	NULL	disulphide-constrained 7-mer	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The peptide is a disulphide-constrained 7-mer with the amino acid sequence CTTMHPRLC that binds to nicotinic acetylcholine receptors .
	manualset3
158658	3	411475	7	NULL	NULL	0	NULL	 amino acid sequence CTTMHPRLC	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The peptide is a disulphide-constrained 7-mer with the amino acid sequence CTTMHPRLC that binds to nicotinic acetylcholine receptors .
	manualset3
158659	4	411475	7	NULL	NULL	0	NULL	nicotinic acetylcholine receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The peptide is a disulphide-constrained 7-mer with the amino acid sequence CTTMHPRLC that binds to nicotinic acetylcholine receptors .
	manualset3
158660	1	411476	7	NULL	NULL	0	NULL	 peptide 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The peptide is secreted from pancreatic beta cells and is thought to have an anti-insulin action .
	manualset3
158661	2	411476	7	NULL	NULL	0	NULL	pancreatic beta cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The peptide is secreted from pancreatic beta cells and is thought to have an anti-insulin action .
	manualset3
158662	3	411476	7	NULL	NULL	0	NULL	anti-insulin action	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The peptide is secreted from pancreatic beta cells and is thought to have an anti-insulin action .
	manualset3
158663	1	411477	7	NULL	NULL	0	NULL	peptide molecular weights ( MWs )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The peptide molecular weights ( MWs ) were analyzed by gel electrophoresis and mass spectrometry , and AAs were quantified by high-performance liquid chromotography .
	manualset3
158664	2	411477	7	NULL	NULL	0	NULL	gel electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The peptide molecular weights ( MWs ) were analyzed by gel electrophoresis and mass spectrometry , and AAs were quantified by high-performance liquid chromotography .
	manualset3
158665	3	411477	7	NULL	NULL	0	NULL	mass spectrometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The peptide molecular weights ( MWs ) were analyzed by gel electrophoresis and mass spectrometry , and AAs were quantified by high-performance liquid chromotography .
	manualset3
158666	4	411477	7	NULL	NULL	0	NULL	AAs	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The peptide molecular weights ( MWs ) were analyzed by gel electrophoresis and mass spectrometry , and AAs were quantified by high-performance liquid chromotography .
	manualset3
158667	5	411477	7	NULL	NULL	0	NULL	high-performance liquid chromotography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The peptide molecular weights ( MWs ) were analyzed by gel electrophoresis and mass spectrometry , and AAs were quantified by high-performance liquid chromotography .
	manualset3
158668	1	411478	7	NULL	NULL	0	NULL	peptide vaccines	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The peptide vaccines induced T-cell responses in the DQ6 mice in which only DQ6 molecules were expressed as MHC class II .
	manualset3
158669	2	411478	7	NULL	NULL	0	NULL	T-cell responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The peptide vaccines induced T-cell responses in the DQ6 mice in which only DQ6 molecules were expressed as MHC class II .
	manualset3
158670	3	411478	7	NULL	NULL	0	NULL	DQ6 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The peptide vaccines induced T-cell responses in the DQ6 mice in which only DQ6 molecules were expressed as MHC class II .
	manualset3
158671	4	411478	7	NULL	NULL	0	NULL	DQ6 molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The peptide vaccines induced T-cell responses in the DQ6 mice in which only DQ6 molecules were expressed as MHC class II .
	manualset3
158672	5	411478	7	NULL	NULL	NULL	NULL	MHC class II	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The peptide vaccines induced T-cell responses in the DQ6 mice in which only DQ6 molecules were expressed as MHC class II .
	manualset3
158673	1	411479	7	NULL	NULL	0	NULL	peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The peptide was successfully folded by zinc treatment and the folded peptide was analyzed intact under neutral conditions by ESI-TOF-MS .
	manualset3
158674	2	411479	7	NULL	NULL	NULL	NULL	zinc treatment	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The peptide was successfully folded by zinc treatment and the folded peptide was analyzed intact under neutral conditions by ESI-TOF-MS .
	manualset3
158675	3	411479	7	NULL	NULL	0	NULL	 folded peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The peptide was successfully folded by zinc treatment and the folded peptide was analyzed intact under neutral conditions by ESI-TOF-MS .
	manualset3
158676	4	411479	7	NULL	NULL	NULL	NULL	neutral conditions	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The peptide was successfully folded by zinc treatment and the folded peptide was analyzed intact under neutral conditions by ESI-TOF-MS .
	manualset3
158677	5	411479	7	NULL	NULL	0	NULL	ESI-TOF-MS 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The peptide was successfully folded by zinc treatment and the folded peptide was analyzed intact under neutral conditions by ESI-TOF-MS .
	manualset3
158678	1	411480	7	NULL	NULL	0	NULL	peptidic opioid delta ( 1 ) agonist ( D-Pen ( 2 ) 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The peptidic opioid delta ( 1 ) agonist ( D-Pen ( 2 ) , D-Pen ( 5 ) ) enkephalin ( DPDPE ) or delta ( 2 ) agonist ( D-Ala ( 2 ) , Glu ( 4 ) ) deltorphin ( DELT ) were given into the rostral-ventral medulla ( RVM ) , intrathecally ( i. th . )
	manualset3
158679	2	411480	7	NULL	NULL	0	NULL	D-Pen ( 5 ) ) enkephalin ( DPDPE )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The peptidic opioid delta ( 1 ) agonist ( D-Pen ( 2 ) , D-Pen ( 5 ) ) enkephalin ( DPDPE ) or delta ( 2 ) agonist ( D-Ala ( 2 ) , Glu ( 4 ) ) deltorphin ( DELT ) were given into the rostral-ventral medulla ( RVM ) , intrathecally ( i. th . )
	manualset3
158680	3	411480	7	NULL	NULL	0	NULL	delta ( 2 ) agonist ( D-Ala ( 2 )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The peptidic opioid delta ( 1 ) agonist ( D-Pen ( 2 ) , D-Pen ( 5 ) ) enkephalin ( DPDPE ) or delta ( 2 ) agonist ( D-Ala ( 2 ) , Glu ( 4 ) ) deltorphin ( DELT ) were given into the rostral-ventral medulla ( RVM ) , intrathecally ( i. th . )
	manualset3
158681	4	411480	7	NULL	NULL	0	NULL	Glu ( 4 ) ) deltorphin ( DELT )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The peptidic opioid delta ( 1 ) agonist ( D-Pen ( 2 ) , D-Pen ( 5 ) ) enkephalin ( DPDPE ) or delta ( 2 ) agonist ( D-Ala ( 2 ) , Glu ( 4 ) ) deltorphin ( DELT ) were given into the rostral-ventral medulla ( RVM ) , intrathecally ( i. th . )
	manualset3
158682	5	411480	7	NULL	NULL	0	NULL	rostral-ventral medulla ( RVM )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The peptidic opioid delta ( 1 ) agonist ( D-Pen ( 2 ) , D-Pen ( 5 ) ) enkephalin ( DPDPE ) or delta ( 2 ) agonist ( D-Ala ( 2 ) , Glu ( 4 ) ) deltorphin ( DELT ) were given into the rostral-ventral medulla ( RVM ) , intrathecally ( i. th . )
	manualset3
158683	6	411480	7	NULL	NULL	0	NULL	intrathecally ( i. th . )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The peptidic opioid delta ( 1 ) agonist ( D-Pen ( 2 ) , D-Pen ( 5 ) ) enkephalin ( DPDPE ) or delta ( 2 ) agonist ( D-Ala ( 2 ) , Glu ( 4 ) ) deltorphin ( DELT ) were given into the rostral-ventral medulla ( RVM ) , intrathecally ( i. th . )
	manualset3
158684	1	411481	7	NULL	NULL	0	NULL	percent change	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The percent change in endothelium-dependent vasodilation at 6 months correlated with the percent change in CRP ( r = -0.44 ; P & lt ; 0.05 ) , but not with changes in plasma lipids .
	manualset3
158685	2	411481	7	NULL	NULL	0	NULL	endothelium-dependent vasodilation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The percent change in endothelium-dependent vasodilation at 6 months correlated with the percent change in CRP ( r = -0.44 ; P & lt ; 0.05 ) , but not with changes in plasma lipids .
	manualset3
158686	3	411481	7	NULL	NULL	0	NULL	6 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The percent change in endothelium-dependent vasodilation at 6 months correlated with the percent change in CRP ( r = -0.44 ; P & lt ; 0.05 ) , but not with changes in plasma lipids .
	manualset3
158687	4	411481	7	NULL	NULL	0	NULL	percent change	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The percent change in endothelium-dependent vasodilation at 6 months correlated with the percent change in CRP ( r = -0.44 ; P & lt ; 0.05 ) , but not with changes in plasma lipids .
	manualset3
158688	5	411481	7	NULL	NULL	NULL	NULL	CRP 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The percent change in endothelium-dependent vasodilation at 6 months correlated with the percent change in CRP ( r = -0.44 ; P & lt ; 0.05 ) , but not with changes in plasma lipids .
	manualset3
158689	6	411481	7	NULL	NULL	0	NULL	( r = -0.44 ; P & lt ; 0.05 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The percent change in endothelium-dependent vasodilation at 6 months correlated with the percent change in CRP ( r = -0.44 ; P & lt ; 0.05 ) , but not with changes in plasma lipids .
	manualset3
158690	7	411481	7	NULL	NULL	0	NULL	plasma lipids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The percent change in endothelium-dependent vasodilation at 6 months correlated with the percent change in CRP ( r = -0.44 ; P & lt ; 0.05 ) , but not with changes in plasma lipids .
	manualset3
158691	1	411482	7	NULL	NULL	0	NULL	percentage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage increase in flow breathing He/O2 was variable ; however , it was similar in normal subjects and in patients with airflow obstruction , and in both groups decreased at low lung volumes .
	manualset3
158692	2	411482	7	NULL	NULL	0	NULL	increase in flow breathing He/O2	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage increase in flow breathing He/O2 was variable ; however , it was similar in normal subjects and in patients with airflow obstruction , and in both groups decreased at low lung volumes .
	manualset3
158694	4	411482	7	NULL	NULL	0	NULL	normal subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage increase in flow breathing He/O2 was variable ; however , it was similar in normal subjects and in patients with airflow obstruction , and in both groups decreased at low lung volumes .
	manualset3
158695	5	411482	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage increase in flow breathing He/O2 was variable ; however , it was similar in normal subjects and in patients with airflow obstruction , and in both groups decreased at low lung volumes .
	manualset3
158696	6	411482	7	NULL	NULL	NULL	NULL	airflow obstruction	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The percentage increase in flow breathing He/O2 was variable ; however , it was similar in normal subjects and in patients with airflow obstruction , and in both groups decreased at low lung volumes .
	manualset3
158697	7	411482	7	NULL	NULL	0	NULL	 groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage increase in flow breathing He/O2 was variable ; however , it was similar in normal subjects and in patients with airflow obstruction , and in both groups decreased at low lung volumes .
	manualset3
158698	8	411482	7	NULL	NULL	0	NULL	low lung volumes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage increase in flow breathing He/O2 was variable ; however , it was similar in normal subjects and in patients with airflow obstruction , and in both groups decreased at low lung volumes .
	manualset3
158699	1	411483	7	NULL	NULL	0	NULL	 percentage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of neurons undergoing necrosis during foetal and early post-natal development in normal and Sprawling ( Swl ) mutant mice was determined .
	manualset3
158700	2	411483	7	NULL	NULL	NULL	NULL	neurons 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The percentage of neurons undergoing necrosis during foetal and early post-natal development in normal and Sprawling ( Swl ) mutant mice was determined .
	manualset3
158701	3	411483	7	NULL	NULL	0	NULL	necrosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of neurons undergoing necrosis during foetal and early post-natal development in normal and Sprawling ( Swl ) mutant mice was determined .
	manualset3
158702	4	411483	7	NULL	NULL	0	NULL	 foetal development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of neurons undergoing necrosis during foetal and early post-natal development in normal and Sprawling ( Swl ) mutant mice was determined .
	manualset3
158703	5	411483	7	NULL	NULL	0	NULL	early post-natal development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of neurons undergoing necrosis during foetal and early post-natal development in normal and Sprawling ( Swl ) mutant mice was determined .
	manualset3
158704	6	411483	7	NULL	NULL	0	NULL	normal mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of neurons undergoing necrosis during foetal and early post-natal development in normal and Sprawling ( Swl ) mutant mice was determined .
	manualset3
158705	7	411483	7	NULL	NULL	0	NULL	Sprawling ( Swl ) mutant mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of neurons undergoing necrosis during foetal and early post-natal development in normal and Sprawling ( Swl ) mutant mice was determined .
	manualset3
158706	1	411484	7	NULL	NULL	0	NULL	percentage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of protein lysine residues which were methylated reached a definite plateau for each temperature , and was considerably increased by heating ( four times at 40 degrees C ) .
	manualset3
158707	2	411484	7	NULL	NULL	0	NULL	protein lysine residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of protein lysine residues which were methylated reached a definite plateau for each temperature , and was considerably increased by heating ( four times at 40 degrees C ) .
	manualset3
158709	4	411484	7	NULL	NULL	0	NULL	definite plateau	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of protein lysine residues which were methylated reached a definite plateau for each temperature , and was considerably increased by heating ( four times at 40 degrees C ) .
	manualset3
158710	5	411484	7	NULL	NULL	NULL	NULL	temperature	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The percentage of protein lysine residues which were methylated reached a definite plateau for each temperature , and was considerably increased by heating ( four times at 40 degrees C ) .
	manualset3
158711	6	411484	7	NULL	NULL	NULL	NULL	 heating	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The percentage of protein lysine residues which were methylated reached a definite plateau for each temperature , and was considerably increased by heating ( four times at 40 degrees C ) .
	manualset3
158712	7	411484	7	NULL	NULL	0	NULL	 four times	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of protein lysine residues which were methylated reached a definite plateau for each temperature , and was considerably increased by heating ( four times at 40 degrees C ) .
	manualset3
158713	8	411484	7	NULL	NULL	0	NULL	40 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of protein lysine residues which were methylated reached a definite plateau for each temperature , and was considerably increased by heating ( four times at 40 degrees C ) .
	manualset3
158714	1	411485	7	NULL	NULL	0	NULL	percentage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of sensitive isolates did not change significantly over time for amoxicillin/clavulanic , cefoxitin , clindamycin and metronidazole .
	manualset3
158715	2	411485	7	NULL	NULL	0	NULL	sensitive isolates	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of sensitive isolates did not change significantly over time for amoxicillin/clavulanic , cefoxitin , clindamycin and metronidazole .
	manualset3
158716	3	411485	7	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of sensitive isolates did not change significantly over time for amoxicillin/clavulanic , cefoxitin , clindamycin and metronidazole .
	manualset3
158717	4	411485	7	NULL	NULL	0	NULL	amoxicillin/clavulanic	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of sensitive isolates did not change significantly over time for amoxicillin/clavulanic , cefoxitin , clindamycin and metronidazole .
	manualset3
158718	5	411485	7	NULL	NULL	0	NULL	cefoxitin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of sensitive isolates did not change significantly over time for amoxicillin/clavulanic , cefoxitin , clindamycin and metronidazole .
	manualset3
158719	6	411485	7	NULL	NULL	0	NULL	clindamycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of sensitive isolates did not change significantly over time for amoxicillin/clavulanic , cefoxitin , clindamycin and metronidazole .
	manualset3
158720	7	411485	7	NULL	NULL	0	NULL	metronidazole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of sensitive isolates did not change significantly over time for amoxicillin/clavulanic , cefoxitin , clindamycin and metronidazole .
	manualset3
158721	1	411486	7	NULL	NULL	0	NULL	 percentage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of total oocysts retained by straining was estimated from effluent mass balance considerations to be 68 % for 710-microm sand , 79 % for 360-microm sand , and 87 % for 150-microm sand .
	manualset3
158722	2	411486	7	NULL	NULL	0	NULL	total oocysts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of total oocysts retained by straining was estimated from effluent mass balance considerations to be 68 % for 710-microm sand , 79 % for 360-microm sand , and 87 % for 150-microm sand .
	manualset3
158723	3	411486	7	NULL	NULL	0	NULL	effluent mass balance	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of total oocysts retained by straining was estimated from effluent mass balance considerations to be 68 % for 710-microm sand , 79 % for 360-microm sand , and 87 % for 150-microm sand .
	manualset3
158724	4	411486	7	NULL	NULL	NULL	NULL	68 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The percentage of total oocysts retained by straining was estimated from effluent mass balance considerations to be 68 % for 710-microm sand , 79 % for 360-microm sand , and 87 % for 150-microm sand .
	manualset3
158725	5	411486	7	NULL	NULL	NULL	NULL	710-microm sand	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The percentage of total oocysts retained by straining was estimated from effluent mass balance considerations to be 68 % for 710-microm sand , 79 % for 360-microm sand , and 87 % for 150-microm sand .
	manualset3
158726	6	411486	7	NULL	NULL	0	NULL	79 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of total oocysts retained by straining was estimated from effluent mass balance considerations to be 68 % for 710-microm sand , 79 % for 360-microm sand , and 87 % for 150-microm sand .
	manualset3
158727	7	411486	7	NULL	NULL	0	NULL	360-microm sand	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of total oocysts retained by straining was estimated from effluent mass balance considerations to be 68 % for 710-microm sand , 79 % for 360-microm sand , and 87 % for 150-microm sand .
	manualset3
158728	8	411486	7	NULL	NULL	0	NULL	 87 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of total oocysts retained by straining was estimated from effluent mass balance considerations to be 68 % for 710-microm sand , 79 % for 360-microm sand , and 87 % for 150-microm sand .
	manualset3
158729	9	411486	7	NULL	NULL	0	NULL	150-microm sand	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of total oocysts retained by straining was estimated from effluent mass balance considerations to be 68 % for 710-microm sand , 79 % for 360-microm sand , and 87 % for 150-microm sand .
	manualset3
158730	1	411487	7	NULL	NULL	0	NULL	percentage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of vinylpyridine moieties quaternized was found to be 35 to 75 % .
	manualset3
158731	2	411487	7	NULL	NULL	0	NULL	 vinylpyridine moieties	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of vinylpyridine moieties quaternized was found to be 35 to 75 % .
	manualset3
158733	3	411487	7	NULL	NULL	NULL	NULL	35 to 75 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The percentage of vinylpyridine moieties quaternized was found to be 35 to 75 % .
	manualset3
158734	1	411488	7	NULL	NULL	0	NULL	percentages 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentages of acetic acid , propionic acid and butyric acid in the fermentation liquids were 68.4 , 25.3 and 6.3 % , respectively , while those in domestic wastewater were 73.0 , 12.2 and 13.8 % , respectively .
	manualset3
158735	2	411488	7	NULL	NULL	0	NULL	acetic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentages of acetic acid , propionic acid and butyric acid in the fermentation liquids were 68.4 , 25.3 and 6.3 % , respectively , while those in domestic wastewater were 73.0 , 12.2 and 13.8 % , respectively .
	manualset3
158736	3	411488	7	NULL	NULL	0	NULL	propionic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentages of acetic acid , propionic acid and butyric acid in the fermentation liquids were 68.4 , 25.3 and 6.3 % , respectively , while those in domestic wastewater were 73.0 , 12.2 and 13.8 % , respectively .
	manualset3
158737	4	411488	7	NULL	NULL	0	NULL	butyric acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentages of acetic acid , propionic acid and butyric acid in the fermentation liquids were 68.4 , 25.3 and 6.3 % , respectively , while those in domestic wastewater were 73.0 , 12.2 and 13.8 % , respectively .
	manualset3
158738	5	411488	7	NULL	NULL	0	NULL	 fermentation liquids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentages of acetic acid , propionic acid and butyric acid in the fermentation liquids were 68.4 , 25.3 and 6.3 % , respectively , while those in domestic wastewater were 73.0 , 12.2 and 13.8 % , respectively .
	manualset3
158739	6	411488	7	NULL	NULL	0	NULL	68.4%	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentages of acetic acid , propionic acid and butyric acid in the fermentation liquids were 68.4 , 25.3 and 6.3 % , respectively , while those in domestic wastewater were 73.0 , 12.2 and 13.8 % , respectively .
	manualset3
158740	7	411488	7	NULL	NULL	0	NULL	25.3%	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentages of acetic acid , propionic acid and butyric acid in the fermentation liquids were 68.4 , 25.3 and 6.3 % , respectively , while those in domestic wastewater were 73.0 , 12.2 and 13.8 % , respectively .
	manualset3
158741	8	411488	7	NULL	NULL	0	NULL	6.3 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentages of acetic acid , propionic acid and butyric acid in the fermentation liquids were 68.4 , 25.3 and 6.3 % , respectively , while those in domestic wastewater were 73.0 , 12.2 and 13.8 % , respectively .
	manualset3
158742	9	411488	7	NULL	NULL	0	NULL	domestic wastewater	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentages of acetic acid , propionic acid and butyric acid in the fermentation liquids were 68.4 , 25.3 and 6.3 % , respectively , while those in domestic wastewater were 73.0 , 12.2 and 13.8 % , respectively .
	manualset3
158743	10	411488	7	NULL	NULL	0	NULL	73.0%	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentages of acetic acid , propionic acid and butyric acid in the fermentation liquids were 68.4 , 25.3 and 6.3 % , respectively , while those in domestic wastewater were 73.0 , 12.2 and 13.8 % , respectively .
	manualset3
158744	11	411488	7	NULL	NULL	0	NULL	12.2%	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentages of acetic acid , propionic acid and butyric acid in the fermentation liquids were 68.4 , 25.3 and 6.3 % , respectively , while those in domestic wastewater were 73.0 , 12.2 and 13.8 % , respectively .
	manualset3
158745	12	411488	7	NULL	NULL	0	NULL	13.8 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentages of acetic acid , propionic acid and butyric acid in the fermentation liquids were 68.4 , 25.3 and 6.3 % , respectively , while those in domestic wastewater were 73.0 , 12.2 and 13.8 % , respectively .
	manualset3
158746	1	411489	7	NULL	NULL	0	NULL	perception of motion smear	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The perception of motion smear during eye and head movements .
	manualset3
158747	2	411489	7	NULL	NULL	0	NULL	eye movements	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The perception of motion smear during eye and head movements .
	manualset3
158748	3	411489	7	NULL	NULL	0	NULL	head movements	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The perception of motion smear during eye and head movements .
	manualset3
158749	1	411490	7	NULL	NULL	NULL	NULL	performance	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The performance of 2C3AB was compared further with the 3ABC fusion protein as the antigen in an indirect ELISA format for DIVA .
	manualset3
158750	2	411490	7	NULL	NULL	0	NULL	2C3AB	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The performance of 2C3AB was compared further with the 3ABC fusion protein as the antigen in an indirect ELISA format for DIVA .
	manualset3
158751	3	411490	7	NULL	NULL	0	NULL	 3ABC fusion protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The performance of 2C3AB was compared further with the 3ABC fusion protein as the antigen in an indirect ELISA format for DIVA .
	manualset3
158752	4	411490	7	NULL	NULL	0	NULL	antigen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The performance of 2C3AB was compared further with the 3ABC fusion protein as the antigen in an indirect ELISA format for DIVA .
	manualset3
158753	5	411490	7	NULL	NULL	0	NULL	 indirect ELISA format	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The performance of 2C3AB was compared further with the 3ABC fusion protein as the antigen in an indirect ELISA format for DIVA .
	manualset3
158754	6	411490	7	NULL	NULL	0	NULL	DIVA	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The performance of 2C3AB was compared further with the 3ABC fusion protein as the antigen in an indirect ELISA format for DIVA .
	manualset3
158755	1	411491	7	NULL	NULL	NULL	NULL	 performance	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The performance of a laboratory-scale BFBR was studied for the treatment of dairy effluent , chosen as a model complex wastewater .
	manualset3
158756	2	411491	7	NULL	NULL	NULL	NULL	laboratory-scale BFBR	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The performance of a laboratory-scale BFBR was studied for the treatment of dairy effluent , chosen as a model complex wastewater .
	manualset3
158757	3	411491	7	NULL	NULL	0	NULL	treatment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The performance of a laboratory-scale BFBR was studied for the treatment of dairy effluent , chosen as a model complex wastewater .
	manualset3
158758	4	411491	7	NULL	NULL	0	NULL	dairy effluent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The performance of a laboratory-scale BFBR was studied for the treatment of dairy effluent , chosen as a model complex wastewater .
	manualset3
158759	5	411491	7	NULL	NULL	0	NULL	model complex wastewater	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The performance of a laboratory-scale BFBR was studied for the treatment of dairy effluent , chosen as a model complex wastewater .
	manualset3
158760	1	411492	7	NULL	NULL	0	NULL	AIB1	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	AIB1 suppressed ROS by up-regulating antioxidants such as glutathione synthetase and glutathione peroxidase , which are targets of the NF-E2-related factor 2 ( Nrf2 ) , a critical transcription factor that regulates antioxidants , detoxification enzymes , and drug efflux proteins .
	manualset3
158761	2	411492	7	NULL	NULL	0	NULL	ROS	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	AIB1 suppressed ROS by up-regulating antioxidants such as glutathione synthetase and glutathione peroxidase , which are targets of the NF-E2-related factor 2 ( Nrf2 ) , a critical transcription factor that regulates antioxidants , detoxification enzymes , and drug efflux proteins .
	manualset3
158762	3	411492	7	NULL	NULL	0	NULL	antioxidants	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	AIB1 suppressed ROS by up-regulating antioxidants such as glutathione synthetase and glutathione peroxidase , which are targets of the NF-E2-related factor 2 ( Nrf2 ) , a critical transcription factor that regulates antioxidants , detoxification enzymes , and drug efflux proteins .
	manualset3
158763	4	411492	7	NULL	NULL	0	NULL	glutathione synthetase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	AIB1 suppressed ROS by up-regulating antioxidants such as glutathione synthetase and glutathione peroxidase , which are targets of the NF-E2-related factor 2 ( Nrf2 ) , a critical transcription factor that regulates antioxidants , detoxification enzymes , and drug efflux proteins .
	manualset3
158764	5	411492	7	NULL	NULL	0	NULL	glutathione peroxidase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	AIB1 suppressed ROS by up-regulating antioxidants such as glutathione synthetase and glutathione peroxidase , which are targets of the NF-E2-related factor 2 ( Nrf2 ) , a critical transcription factor that regulates antioxidants , detoxification enzymes , and drug efflux proteins .
	manualset3
158765	6	411492	7	NULL	NULL	NULL	NULL	NF-E2-related factor 2 ( Nrf2 )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	AIB1 suppressed ROS by up-regulating antioxidants such as glutathione synthetase and glutathione peroxidase , which are targets of the NF-E2-related factor 2 ( Nrf2 ) , a critical transcription factor that regulates antioxidants , detoxification enzymes , and drug efflux proteins .
	manualset3
158766	7	411492	7	NULL	NULL	0	NULL	transcription factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	AIB1 suppressed ROS by up-regulating antioxidants such as glutathione synthetase and glutathione peroxidase , which are targets of the NF-E2-related factor 2 ( Nrf2 ) , a critical transcription factor that regulates antioxidants , detoxification enzymes , and drug efflux proteins .
	manualset3
158767	8	411492	7	NULL	NULL	0	NULL	antioxidants	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	AIB1 suppressed ROS by up-regulating antioxidants such as glutathione synthetase and glutathione peroxidase , which are targets of the NF-E2-related factor 2 ( Nrf2 ) , a critical transcription factor that regulates antioxidants , detoxification enzymes , and drug efflux proteins .
	manualset3
158768	9	411492	7	NULL	NULL	0	NULL	detoxification enzymes	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	AIB1 suppressed ROS by up-regulating antioxidants such as glutathione synthetase and glutathione peroxidase , which are targets of the NF-E2-related factor 2 ( Nrf2 ) , a critical transcription factor that regulates antioxidants , detoxification enzymes , and drug efflux proteins .
	manualset3
158769	10	411492	7	NULL	NULL	0	NULL	drug efflux proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	AIB1 suppressed ROS by up-regulating antioxidants such as glutathione synthetase and glutathione peroxidase , which are targets of the NF-E2-related factor 2 ( Nrf2 ) , a critical transcription factor that regulates antioxidants , detoxification enzymes , and drug efflux proteins .
	manualset3
158770	11	411492	7	NULL	NULL	NULL	NULL	targets	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	AIB1 suppressed ROS by up-regulating antioxidants such as glutathione synthetase and glutathione peroxidase , which are targets of the NF-E2-related factor 2 ( Nrf2 ) , a critical transcription factor that regulates antioxidants , detoxification enzymes , and drug efflux proteins .
	manualset3
158771	1	411493	7	NULL	NULL	0	NULL	performance	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The performance of the qPCR assay and of the overall CBPV quantitation method were validated over a 6 log range from 10 ( 2 ) to 10 ( 8 ) with a detection limit of 50 and 100 CBPV RNA copies , respectively , and the protocol of the real-time RT-qPCR assay for CBPV quantitation was approved by the French Accreditation Committee .
	manualset3
158772	2	411493	7	NULL	NULL	0	NULL	qPCR assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The performance of the qPCR assay and of the overall CBPV quantitation method were validated over a 6 log range from 10 ( 2 ) to 10 ( 8 ) with a detection limit of 50 and 100 CBPV RNA copies , respectively , and the protocol of the real-time RT-qPCR assay for CBPV quantitation was approved by the French Accreditation Committee .
	manualset3
158773	3	411493	7	NULL	NULL	0	NULL	 overall CBPV quantitation method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The performance of the qPCR assay and of the overall CBPV quantitation method were validated over a 6 log range from 10 ( 2 ) to 10 ( 8 ) with a detection limit of 50 and 100 CBPV RNA copies , respectively , and the protocol of the real-time RT-qPCR assay for CBPV quantitation was approved by the French Accreditation Committee .
	manualset3
158774	4	411493	7	NULL	NULL	NULL	NULL	6 log range	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The performance of the qPCR assay and of the overall CBPV quantitation method were validated over a 6 log range from 10 ( 2 ) to 10 ( 8 ) with a detection limit of 50 and 100 CBPV RNA copies , respectively , and the protocol of the real-time RT-qPCR assay for CBPV quantitation was approved by the French Accreditation Committee .
	manualset3
158775	5	411493	7	NULL	NULL	0	NULL	10 ( 2 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The performance of the qPCR assay and of the overall CBPV quantitation method were validated over a 6 log range from 10 ( 2 ) to 10 ( 8 ) with a detection limit of 50 and 100 CBPV RNA copies , respectively , and the protocol of the real-time RT-qPCR assay for CBPV quantitation was approved by the French Accreditation Committee .
	manualset3
158776	6	411493	7	NULL	NULL	0	NULL	10 ( 8 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The performance of the qPCR assay and of the overall CBPV quantitation method were validated over a 6 log range from 10 ( 2 ) to 10 ( 8 ) with a detection limit of 50 and 100 CBPV RNA copies , respectively , and the protocol of the real-time RT-qPCR assay for CBPV quantitation was approved by the French Accreditation Committee .
	manualset3
158777	7	411493	7	NULL	NULL	0	NULL	detection limit 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The performance of the qPCR assay and of the overall CBPV quantitation method were validated over a 6 log range from 10 ( 2 ) to 10 ( 8 ) with a detection limit of 50 and 100 CBPV RNA copies , respectively , and the protocol of the real-time RT-qPCR assay for CBPV quantitation was approved by the French Accreditation Committee .
	manualset3
158778	8	411493	7	NULL	NULL	0	NULL	50 and 100 CBPV RNA copies	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The performance of the qPCR assay and of the overall CBPV quantitation method were validated over a 6 log range from 10 ( 2 ) to 10 ( 8 ) with a detection limit of 50 and 100 CBPV RNA copies , respectively , and the protocol of the real-time RT-qPCR assay for CBPV quantitation was approved by the French Accreditation Committee .
	manualset3
158779	9	411493	7	NULL	NULL	0	NULL	protocol	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The performance of the qPCR assay and of the overall CBPV quantitation method were validated over a 6 log range from 10 ( 2 ) to 10 ( 8 ) with a detection limit of 50 and 100 CBPV RNA copies , respectively , and the protocol of the real-time RT-qPCR assay for CBPV quantitation was approved by the French Accreditation Committee .
	manualset3
158780	10	411493	7	NULL	NULL	0	NULL	 real-time RT-qPCR assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The performance of the qPCR assay and of the overall CBPV quantitation method were validated over a 6 log range from 10 ( 2 ) to 10 ( 8 ) with a detection limit of 50 and 100 CBPV RNA copies , respectively , and the protocol of the real-time RT-qPCR assay for CBPV quantitation was approved by the French Accreditation Committee .
	manualset3
158781	11	411493	7	NULL	NULL	0	NULL	CBPV quantitation	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The performance of the qPCR assay and of the overall CBPV quantitation method were validated over a 6 log range from 10 ( 2 ) to 10 ( 8 ) with a detection limit of 50 and 100 CBPV RNA copies , respectively , and the protocol of the real-time RT-qPCR assay for CBPV quantitation was approved by the French Accreditation Committee .
	manualset3
158782	12	411493	7	NULL	NULL	NULL	NULL	French Accreditation Committee 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The performance of the qPCR assay and of the overall CBPV quantitation method were validated over a 6 log range from 10 ( 2 ) to 10 ( 8 ) with a detection limit of 50 and 100 CBPV RNA copies , respectively , and the protocol of the real-time RT-qPCR assay for CBPV quantitation was approved by the French Accreditation Committee .
	manualset3
158783	1	411494	7	NULL	NULL	0	NULL	pericytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The pericytes were situated away from the endothelial cells .
	manualset3
158784	2	411494	7	NULL	NULL	0	NULL	endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The pericytes were situated away from the endothelial cells .
	manualset3
158785	1	411495	7	NULL	NULL	NULL	NULL	perinatal mortality 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The perinatal mortality was 17/1000 .
	manualset3
158786	2	411495	7	NULL	NULL	0	NULL	17/1000	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The perinatal mortality was 17/1000 .
	manualset3
158787	1	411496	7	NULL	NULL	0	NULL	permeability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The permeability of lysosomes to sugars .
	manualset3
158788	2	411496	7	NULL	NULL	0	NULL	 lysosomes 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The permeability of lysosomes to sugars .
	manualset3
158789	3	411496	7	NULL	NULL	0	NULL	sugars	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The permeability of lysosomes to sugars .
	manualset3
158790	1	411497	7	NULL	NULL	0	NULL	persistence of AV block 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The persistence of AV block after a 3-month detraining period led us to believe that our decision was reasonable .
	manualset3
158791	2	411497	7	NULL	NULL	0	NULL	3 month	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The persistence of AV block after a 3-month detraining period led us to believe that our decision was reasonable .
	manualset3
158792	3	411497	7	NULL	NULL	0	NULL	detraining period	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The persistence of AV block after a 3-month detraining period led us to believe that our decision was reasonable .
	manualset3
158793	4	411497	7	NULL	NULL	0	NULL	decision	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The persistence of AV block after a 3-month detraining period led us to believe that our decision was reasonable .
	manualset3
158794	1	411498	7	NULL	NULL	0	NULL	persistence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The persistence of `` steroid-synthesizing cell '' antigen and 3beta-hydroxysteroid dehydrogenase in organ cultures of normal human placentas .
	manualset3
158795	2	411498	7	NULL	NULL	0	NULL	steroid-synthesizing cell 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The persistence of `` steroid-synthesizing cell '' antigen and 3beta-hydroxysteroid dehydrogenase in organ cultures of normal human placentas .
	manualset3
158796	3	411498	7	NULL	NULL	0	NULL	antigen 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The persistence of `` steroid-synthesizing cell '' antigen and 3beta-hydroxysteroid dehydrogenase in organ cultures of normal human placentas .
	manualset3
158797	4	411498	7	NULL	NULL	0	NULL	3beta-hydroxysteroid dehydrogenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The persistence of `` steroid-synthesizing cell '' antigen and 3beta-hydroxysteroid dehydrogenase in organ cultures of normal human placentas .
	manualset3
158798	5	411498	7	NULL	NULL	0	NULL	organ cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The persistence of `` steroid-synthesizing cell '' antigen and 3beta-hydroxysteroid dehydrogenase in organ cultures of normal human placentas .
	manualset3
158799	6	411498	7	NULL	NULL	0	NULL	normal human placentas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The persistence of `` steroid-synthesizing cell '' antigen and 3beta-hydroxysteroid dehydrogenase in organ cultures of normal human placentas .
	manualset3
158800	1	411499	7	NULL	NULL	0	NULL	persistence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The persistence of motor unit potentials with late components is taken to imply that the late components were caused either by sprouts that failed to undergo myelination or , more likely , by ectopically innervated muscle fibers .
	manualset3
158801	2	411499	7	NULL	NULL	0	NULL	motor unit potentials	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The persistence of motor unit potentials with late components is taken to imply that the late components were caused either by sprouts that failed to undergo myelination or , more likely , by ectopically innervated muscle fibers .
	manualset3
158802	3	411499	7	NULL	NULL	0	NULL	late components	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The persistence of motor unit potentials with late components is taken to imply that the late components were caused either by sprouts that failed to undergo myelination or , more likely , by ectopically innervated muscle fibers .
	manualset3
158803	4	411499	7	NULL	NULL	0	NULL	late components	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The persistence of motor unit potentials with late components is taken to imply that the late components were caused either by sprouts that failed to undergo myelination or , more likely , by ectopically innervated muscle fibers .
	manualset3
158804	5	411499	7	NULL	NULL	0	NULL	sprouts	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The persistence of motor unit potentials with late components is taken to imply that the late components were caused either by sprouts that failed to undergo myelination or , more likely , by ectopically innervated muscle fibers .
	manualset3
158805	6	411499	7	NULL	NULL	0	NULL	myelination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The persistence of motor unit potentials with late components is taken to imply that the late components were caused either by sprouts that failed to undergo myelination or , more likely , by ectopically innervated muscle fibers .
	manualset3
158806	7	411499	7	NULL	NULL	0	NULL	ectopically innervated muscle fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The persistence of motor unit potentials with late components is taken to imply that the late components were caused either by sprouts that failed to undergo myelination or , more likely , by ectopically innervated muscle fibers .
	manualset3
158807	1	411500	7	NULL	NULL	0	NULL	persistence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The persistence or loss of IgG and IgM antibody specificities for individual polypeptides of Treponema pallidum after therapy for syphilis was examined by sodium dodecyl sulfate-polyacrylamide gel electrophoresis ( SDS-PAGE ) and by the Western blot technique .
	manualset3
158808	2	411500	7	NULL	NULL	0	NULL	loss of IgG antibody specificities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The persistence or loss of IgG and IgM antibody specificities for individual polypeptides of Treponema pallidum after therapy for syphilis was examined by sodium dodecyl sulfate-polyacrylamide gel electrophoresis ( SDS-PAGE ) and by the Western blot technique .
	manualset3
158809	3	411500	7	NULL	NULL	0	NULL	IgM antibody specificities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The persistence or loss of IgG and IgM antibody specificities for individual polypeptides of Treponema pallidum after therapy for syphilis was examined by sodium dodecyl sulfate-polyacrylamide gel electrophoresis ( SDS-PAGE ) and by the Western blot technique .
	manualset3
158810	4	411500	7	NULL	NULL	0	NULL	 individual polypeptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The persistence or loss of IgG and IgM antibody specificities for individual polypeptides of Treponema pallidum after therapy for syphilis was examined by sodium dodecyl sulfate-polyacrylamide gel electrophoresis ( SDS-PAGE ) and by the Western blot technique .
	manualset3
158811	5	411500	7	NULL	NULL	0	NULL	Treponema pallidum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The persistence or loss of IgG and IgM antibody specificities for individual polypeptides of Treponema pallidum after therapy for syphilis was examined by sodium dodecyl sulfate-polyacrylamide gel electrophoresis ( SDS-PAGE ) and by the Western blot technique .
	manualset3
158812	6	411500	7	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The persistence or loss of IgG and IgM antibody specificities for individual polypeptides of Treponema pallidum after therapy for syphilis was examined by sodium dodecyl sulfate-polyacrylamide gel electrophoresis ( SDS-PAGE ) and by the Western blot technique .
	manualset3
158813	7	411500	7	NULL	NULL	NULL	NULL	syphilis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The persistence or loss of IgG and IgM antibody specificities for individual polypeptides of Treponema pallidum after therapy for syphilis was examined by sodium dodecyl sulfate-polyacrylamide gel electrophoresis ( SDS-PAGE ) and by the Western blot technique .
	manualset3
158814	8	411500	7	NULL	NULL	0	NULL	sodium dodecyl sulfate-polyacrylamide gel electrophoresis ( SDS-PAGE ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The persistence or loss of IgG and IgM antibody specificities for individual polypeptides of Treponema pallidum after therapy for syphilis was examined by sodium dodecyl sulfate-polyacrylamide gel electrophoresis ( SDS-PAGE ) and by the Western blot technique .
	manualset3
158815	9	411500	7	NULL	NULL	0	NULL	Western blot technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The persistence or loss of IgG and IgM antibody specificities for individual polypeptides of Treponema pallidum after therapy for syphilis was examined by sodium dodecyl sulfate-polyacrylamide gel electrophoresis ( SDS-PAGE ) and by the Western blot technique .
	manualset3
158816	1	411501	7	NULL	NULL	0	NULL	AIDS-related opportunistic infections 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	AIDS-related opportunistic infections of the central nervous system are discussed , presenting both a review of the literature and several case reports .
	manualset3
158817	2	411501	7	NULL	NULL	0	NULL	central nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	AIDS-related opportunistic infections of the central nervous system are discussed , presenting both a review of the literature and several case reports .
	manualset3
158818	3	411501	7	NULL	NULL	0	NULL	review of the literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	AIDS-related opportunistic infections of the central nervous system are discussed , presenting both a review of the literature and several case reports .
	manualset3
158819	4	411501	7	NULL	NULL	0	NULL	several case reports	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	AIDS-related opportunistic infections of the central nervous system are discussed , presenting both a review of the literature and several case reports .
	manualset3
158820	1	411502	7	NULL	NULL	0	NULL	personal and interpersonal significance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The personal and interpersonal significance of menarche .
	manualset3
158821	2	411502	7	NULL	NULL	0	NULL	menarche 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The personal and interpersonal significance of menarche .
	manualset3
158822	1	411503	7	NULL	NULL	0	NULL	pesticide residues	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The pesticide residues were found in the order sigmaDDT ) Heptachlor ) Dieldrin ) Aldrin .
	manualset3
158823	2	411503	7	NULL	NULL	0	NULL	order	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The pesticide residues were found in the order sigmaDDT ) Heptachlor ) Dieldrin ) Aldrin .
	manualset3
158824	3	411503	7	NULL	NULL	0	NULL	sigmaDDT	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The pesticide residues were found in the order sigmaDDT ) Heptachlor ) Dieldrin ) Aldrin .
	manualset3
158825	4	411503	7	NULL	NULL	0	NULL	Heptachlor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The pesticide residues were found in the order sigmaDDT ) Heptachlor ) Dieldrin ) Aldrin .
	manualset3
158826	5	411503	7	NULL	NULL	0	NULL	Dieldrin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The pesticide residues were found in the order sigmaDDT ) Heptachlor ) Dieldrin ) Aldrin .
	manualset3
158827	6	411503	7	NULL	NULL	0	NULL	Aldrin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The pesticide residues were found in the order sigmaDDT ) Heptachlor ) Dieldrin ) Aldrin .
	manualset3
158828	1	411504	7	NULL	NULL	0	NULL	phantom pains	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The phantom pains were described as either pricking and shooting or like hemorrhoids or hard stools that would rupture the rectum .
	manualset3
158829	2	411504	7	NULL	NULL	0	NULL	pricking	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The phantom pains were described as either pricking and shooting or like hemorrhoids or hard stools that would rupture the rectum .
	manualset3
158830	3	411504	7	NULL	NULL	0	NULL	shooting	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The phantom pains were described as either pricking and shooting or like hemorrhoids or hard stools that would rupture the rectum .
	manualset3
158831	4	411504	7	NULL	NULL	0	NULL	hemorrhoids	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The phantom pains were described as either pricking and shooting or like hemorrhoids or hard stools that would rupture the rectum .
	manualset3
158832	5	411504	7	NULL	NULL	0	NULL	hard stools	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The phantom pains were described as either pricking and shooting or like hemorrhoids or hard stools that would rupture the rectum .
	manualset3
158833	6	411504	7	NULL	NULL	0	NULL	rectum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The phantom pains were described as either pricking and shooting or like hemorrhoids or hard stools that would rupture the rectum .
	manualset3
158834	1	411505	7	NULL	NULL	0	NULL	pharmacokinetic profiles	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The pharmacokinetic profiles of these three ACE inhibitors differ .
	manualset3
158835	2	411505	7	NULL	NULL	0	NULL	three ACE inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The pharmacokinetic profiles of these three ACE inhibitors differ .
	manualset3
158836	1	411506	7	NULL	NULL	0	NULL	pharmacokinetics 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The pharmacokinetics of ceftizoxime ( FK-749 ) were studied in 20 volunteers with various degrees of renal function .
	manualset3
158837	2	411506	7	NULL	NULL	0	NULL	ceftizoxime ( FK-749 )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The pharmacokinetics of ceftizoxime ( FK-749 ) were studied in 20 volunteers with various degrees of renal function .
	manualset3
158838	3	411506	7	NULL	NULL	0	NULL	20 volunteers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The pharmacokinetics of ceftizoxime ( FK-749 ) were studied in 20 volunteers with various degrees of renal function .
	manualset3
158839	4	411506	7	NULL	NULL	NULL	NULL	various degrees 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The pharmacokinetics of ceftizoxime ( FK-749 ) were studied in 20 volunteers with various degrees of renal function .
	manualset3
159410	5	411506	7	NULL	NULL	0	NULL	renal function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The pharmacokinetics of ceftizoxime ( FK-749 ) were studied in 20 volunteers with various degrees of renal function .
	manualset3
158840	1	411507	7	NULL	NULL	NULL	NULL	pharmacokinetics	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The pharmacokinetics of riluzole , determined on the morning of the 5th day of dosing , were not significantly affected by age or gender .
	manualset3
158841	2	411507	7	NULL	NULL	0	NULL	riluzole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The pharmacokinetics of riluzole , determined on the morning of the 5th day of dosing , were not significantly affected by age or gender .
	manualset3
158842	3	411507	7	NULL	NULL	0	NULL	morning 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The pharmacokinetics of riluzole , determined on the morning of the 5th day of dosing , were not significantly affected by age or gender .
	manualset3
158843	4	411507	7	NULL	NULL	0	NULL	 5th day	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The pharmacokinetics of riluzole , determined on the morning of the 5th day of dosing , were not significantly affected by age or gender .
	manualset3
158844	5	411507	7	NULL	NULL	0	NULL	dosing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The pharmacokinetics of riluzole , determined on the morning of the 5th day of dosing , were not significantly affected by age or gender .
	manualset3
158845	6	411507	7	NULL	NULL	0	NULL	age	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The pharmacokinetics of riluzole , determined on the morning of the 5th day of dosing , were not significantly affected by age or gender .
	manualset3
158846	7	411507	7	NULL	NULL	0	NULL	gender	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The pharmacokinetics of riluzole , determined on the morning of the 5th day of dosing , were not significantly affected by age or gender .
	manualset3
158847	1	411508	7	NULL	NULL	0	NULL	AII	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	AII binds to specific cell surface receptors present on a number of different renal cell types including mesangial , vascular smooth muscle , tubular and interstitial cells , and activates many of the intracellular signalling pathways associated with cell growth .
	manualset3
158848	2	411508	7	NULL	NULL	0	NULL	cell surface receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	AII binds to specific cell surface receptors present on a number of different renal cell types including mesangial , vascular smooth muscle , tubular and interstitial cells , and activates many of the intracellular signalling pathways associated with cell growth .
	manualset3
158849	3	411508	7	NULL	NULL	NULL	NULL	renal cell types	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	AII binds to specific cell surface receptors present on a number of different renal cell types including mesangial , vascular smooth muscle , tubular and interstitial cells , and activates many of the intracellular signalling pathways associated with cell growth .
	manualset3
158850	4	411508	7	NULL	NULL	0	NULL	mesangial cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	AII binds to specific cell surface receptors present on a number of different renal cell types including mesangial , vascular smooth muscle , tubular and interstitial cells , and activates many of the intracellular signalling pathways associated with cell growth .
	manualset3
158851	5	411508	7	NULL	NULL	0	NULL	 vascular smooth muscle cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	AII binds to specific cell surface receptors present on a number of different renal cell types including mesangial , vascular smooth muscle , tubular and interstitial cells , and activates many of the intracellular signalling pathways associated with cell growth .
	manualset3
158852	6	411508	7	NULL	NULL	0	NULL	tubular and interstitial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	AII binds to specific cell surface receptors present on a number of different renal cell types including mesangial , vascular smooth muscle , tubular and interstitial cells , and activates many of the intracellular signalling pathways associated with cell growth .
	manualset3
158853	7	411508	7	NULL	NULL	0	NULL	intracellular signalling pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	AII binds to specific cell surface receptors present on a number of different renal cell types including mesangial , vascular smooth muscle , tubular and interstitial cells , and activates many of the intracellular signalling pathways associated with cell growth .
	manualset3
158854	8	411508	7	NULL	NULL	0	NULL	cell growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	AII binds to specific cell surface receptors present on a number of different renal cell types including mesangial , vascular smooth muscle , tubular and interstitial cells , and activates many of the intracellular signalling pathways associated with cell growth .
	manualset3
159411	9	411508	7	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	AII binds to specific cell surface receptors present on a number of different renal cell types including mesangial , vascular smooth muscle , tubular and interstitial cells , and activates many of the intracellular signalling pathways associated with cell growth .
	manualset3
158855	1	411509	7	NULL	NULL	0	NULL	pharmacological effect	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The pharmacological effect was not produced through the stimulation of cyclooxygenase , adenyl cyclase , or guanylyl cyclase , since selective inhibitors did not prevent the fraction S4-induced effects .
	manualset3
158856	2	411509	7	NULL	NULL	0	NULL	 stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The pharmacological effect was not produced through the stimulation of cyclooxygenase , adenyl cyclase , or guanylyl cyclase , since selective inhibitors did not prevent the fraction S4-induced effects .
	manualset3
158857	3	411509	7	NULL	NULL	0	NULL	cyclooxygenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The pharmacological effect was not produced through the stimulation of cyclooxygenase , adenyl cyclase , or guanylyl cyclase , since selective inhibitors did not prevent the fraction S4-induced effects .
	manualset3
158858	4	411509	7	NULL	NULL	0	NULL	adenyl cyclase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The pharmacological effect was not produced through the stimulation of cyclooxygenase , adenyl cyclase , or guanylyl cyclase , since selective inhibitors did not prevent the fraction S4-induced effects .
	manualset3
158859	5	411509	7	NULL	NULL	0	NULL	guanylyl cyclase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The pharmacological effect was not produced through the stimulation of cyclooxygenase , adenyl cyclase , or guanylyl cyclase , since selective inhibitors did not prevent the fraction S4-induced effects .
	manualset3
158860	6	411509	7	NULL	NULL	0	NULL	selective inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The pharmacological effect was not produced through the stimulation of cyclooxygenase , adenyl cyclase , or guanylyl cyclase , since selective inhibitors did not prevent the fraction S4-induced effects .
	manualset3
158861	7	411509	7	NULL	NULL	0	NULL	fraction S4-induced effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The pharmacological effect was not produced through the stimulation of cyclooxygenase , adenyl cyclase , or guanylyl cyclase , since selective inhibitors did not prevent the fraction S4-induced effects .
	manualset3
158862	1	411510	7	NULL	NULL	NULL	NULL	 pharmacological inhibition 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The pharmacological inhibition of phosphoinositide 3-kinase ( PI3K ) , an upstream kinase responsible for Akt phosphorylation , abrogated cis-GS-induced Nrf2 nuclear translocation .
	manualset3
158863	2	411510	7	NULL	NULL	0	NULL	phosphoinositide 3-kinase ( PI3K )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The pharmacological inhibition of phosphoinositide 3-kinase ( PI3K ) , an upstream kinase responsible for Akt phosphorylation , abrogated cis-GS-induced Nrf2 nuclear translocation .
	manualset3
158864	3	411510	7	NULL	NULL	0	NULL	upstream kinase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The pharmacological inhibition of phosphoinositide 3-kinase ( PI3K ) , an upstream kinase responsible for Akt phosphorylation , abrogated cis-GS-induced Nrf2 nuclear translocation .
	manualset3
158865	4	411510	7	NULL	NULL	NULL	NULL	Akt phosphorylation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The pharmacological inhibition of phosphoinositide 3-kinase ( PI3K ) , an upstream kinase responsible for Akt phosphorylation , abrogated cis-GS-induced Nrf2 nuclear translocation .
	manualset3
158866	5	411510	7	NULL	NULL	NULL	NULL	 cis-GS-induced Nrf2 nuclear translocation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The pharmacological inhibition of phosphoinositide 3-kinase ( PI3K ) , an upstream kinase responsible for Akt phosphorylation , abrogated cis-GS-induced Nrf2 nuclear translocation .
	manualset3
158867	1	411511	7	NULL	NULL	0	NULL	pharmacy department 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The pharmacy department planned to issue bulletins designed to correct the problems .
	manualset3
158868	2	411511	7	NULL	NULL	0	NULL	bulletins	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The pharmacy department planned to issue bulletins designed to correct the problems .
	manualset3
158869	3	411511	7	NULL	NULL	0	NULL	problems	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The pharmacy department planned to issue bulletins designed to correct the problems .
	manualset3
158870	1	411512	7	NULL	NULL	0	NULL	phenomenon 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The phenomenon of concurrent pain in craniofacial and cervical structures is considered , and clinical reports and opinions are presented regarding theories of cervical-to-craniofacial and craniofacial-to-cervical pain referral .
	manualset3
158871	2	411512	7	NULL	NULL	0	NULL	concurrent pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The phenomenon of concurrent pain in craniofacial and cervical structures is considered , and clinical reports and opinions are presented regarding theories of cervical-to-craniofacial and craniofacial-to-cervical pain referral .
	manualset3
158872	3	411512	7	NULL	NULL	0	NULL	craniofacial structure	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The phenomenon of concurrent pain in craniofacial and cervical structures is considered , and clinical reports and opinions are presented regarding theories of cervical-to-craniofacial and craniofacial-to-cervical pain referral .
	manualset3
158873	4	411512	7	NULL	NULL	0	NULL	cervical structures	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The phenomenon of concurrent pain in craniofacial and cervical structures is considered , and clinical reports and opinions are presented regarding theories of cervical-to-craniofacial and craniofacial-to-cervical pain referral .
	manualset3
158874	5	411512	7	NULL	NULL	0	NULL	clinical reports	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The phenomenon of concurrent pain in craniofacial and cervical structures is considered , and clinical reports and opinions are presented regarding theories of cervical-to-craniofacial and craniofacial-to-cervical pain referral .
	manualset3
158875	6	411512	7	NULL	NULL	NULL	NULL	opinions	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The phenomenon of concurrent pain in craniofacial and cervical structures is considered , and clinical reports and opinions are presented regarding theories of cervical-to-craniofacial and craniofacial-to-cervical pain referral .
	manualset3
158876	7	411512	7	NULL	NULL	0	NULL	 theories	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The phenomenon of concurrent pain in craniofacial and cervical structures is considered , and clinical reports and opinions are presented regarding theories of cervical-to-craniofacial and craniofacial-to-cervical pain referral .
	manualset3
158877	8	411512	7	NULL	NULL	0	NULL	cervical-to-craniofacial pain referral	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The phenomenon of concurrent pain in craniofacial and cervical structures is considered , and clinical reports and opinions are presented regarding theories of cervical-to-craniofacial and craniofacial-to-cervical pain referral .
	manualset3
158878	9	411512	7	NULL	NULL	0	NULL	craniofacial-to-cervical pain referral	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The phenomenon of concurrent pain in craniofacial and cervical structures is considered , and clinical reports and opinions are presented regarding theories of cervical-to-craniofacial and craniofacial-to-cervical pain referral .
	manualset3
158879	1	411513	7	NULL	NULL	0	NULL	phenotype	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The phenotype of WIL varied drastically from patient to patient , as determined by their expression of CD4 , CD8 , T-cell receptor alpha/beta chain ( TCR alpha beta ) , and TCR gamma delta .
	manualset3
158880	2	411513	7	NULL	NULL	0	NULL	WIL	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The phenotype of WIL varied drastically from patient to patient , as determined by their expression of CD4 , CD8 , T-cell receptor alpha/beta chain ( TCR alpha beta ) , and TCR gamma delta .
	manualset3
158881	3	411513	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The phenotype of WIL varied drastically from patient to patient , as determined by their expression of CD4 , CD8 , T-cell receptor alpha/beta chain ( TCR alpha beta ) , and TCR gamma delta .
	manualset3
158882	4	411513	7	NULL	NULL	0	NULL	 patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The phenotype of WIL varied drastically from patient to patient , as determined by their expression of CD4 , CD8 , T-cell receptor alpha/beta chain ( TCR alpha beta ) , and TCR gamma delta .
	manualset3
158883	5	411513	7	NULL	NULL	NULL	NULL	expression of CD4	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The phenotype of WIL varied drastically from patient to patient , as determined by their expression of CD4 , CD8 , T-cell receptor alpha/beta chain ( TCR alpha beta ) , and TCR gamma delta .
	manualset3
158884	6	411513	7	NULL	NULL	NULL	NULL	expression of CD8	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The phenotype of WIL varied drastically from patient to patient , as determined by their expression of CD4 , CD8 , T-cell receptor alpha/beta chain ( TCR alpha beta ) , and TCR gamma delta .
	manualset3
158885	7	411513	7	NULL	NULL	NULL	NULL	expression of T-cell receptor alpha/beta chain ( TCR alpha beta ) 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The phenotype of WIL varied drastically from patient to patient , as determined by their expression of CD4 , CD8 , T-cell receptor alpha/beta chain ( TCR alpha beta ) , and TCR gamma delta .
	manualset3
158886	8	411513	7	NULL	NULL	NULL	NULL	expression of TCR gamma delta	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The phenotype of WIL varied drastically from patient to patient , as determined by their expression of CD4 , CD8 , T-cell receptor alpha/beta chain ( TCR alpha beta ) , and TCR gamma delta .
	manualset3
158887	1	411514	7	NULL	NULL	0	NULL	phosphate group	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The phosphate group is connected via intramolecular hydrogen bonds to coordinated water molecules .
	manualset3
158888	2	411514	7	NULL	NULL	0	NULL	intramolecular hydrogen bonds	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The phosphate group is connected via intramolecular hydrogen bonds to coordinated water molecules .
	manualset3
158889	3	411514	7	NULL	NULL	0	NULL	water molecules	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The phosphate group is connected via intramolecular hydrogen bonds to coordinated water molecules .
	manualset3
158890	1	411515	7	NULL	NULL	NULL	NULL	phosphate transporter , Pho84p	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The phosphate transporter , Pho84p , known to import arsenate , was overexpressed using a 2-based vector carrying PHO84 under the control of the late-phase ADH2 promoter .
	manualset3
158891	2	411515	7	NULL	NULL	0	NULL	arsenate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The phosphate transporter , Pho84p , known to import arsenate , was overexpressed using a 2-based vector carrying PHO84 under the control of the late-phase ADH2 promoter .
	manualset3
158892	3	411515	7	NULL	NULL	0	NULL	2-based vector	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The phosphate transporter , Pho84p , known to import arsenate , was overexpressed using a 2-based vector carrying PHO84 under the control of the late-phase ADH2 promoter .
	manualset3
158893	4	411515	7	NULL	NULL	0	NULL	PHO84	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The phosphate transporter , Pho84p , known to import arsenate , was overexpressed using a 2-based vector carrying PHO84 under the control of the late-phase ADH2 promoter .
	manualset3
158894	5	411515	7	NULL	NULL	0	NULL	control	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The phosphate transporter , Pho84p , known to import arsenate , was overexpressed using a 2-based vector carrying PHO84 under the control of the late-phase ADH2 promoter .
	manualset3
158895	6	411515	7	NULL	NULL	0	NULL	late-phase ADH2 promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The phosphate transporter , Pho84p , known to import arsenate , was overexpressed using a 2-based vector carrying PHO84 under the control of the late-phase ADH2 promoter .
	manualset3
158896	1	411516	7	NULL	NULL	0	NULL	 phospholipids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The phospholipids from human thyroid have been identified and determined by two-dimensional chromatography .
	manualset3
158897	2	411516	7	NULL	NULL	0	NULL	human thyroid	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The phospholipids from human thyroid have been identified and determined by two-dimensional chromatography .
	manualset3
158898	3	411516	7	NULL	NULL	0	NULL	two-dimensional chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The phospholipids from human thyroid have been identified and determined by two-dimensional chromatography .
	manualset3
158899	1	411517	7	NULL	NULL	0	NULL	AKAP79/150	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	AKAP79/150 is targeted to dendritic spine plasma membranes by an N-terminal polybasic domain that binds phosphoinositide lipids , F-actin , and cadherin cell adhesion molecules .
	manualset3
158900	2	411517	7	NULL	NULL	0	NULL	dendritic spine plasma membranes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	AKAP79/150 is targeted to dendritic spine plasma membranes by an N-terminal polybasic domain that binds phosphoinositide lipids , F-actin , and cadherin cell adhesion molecules .
	manualset3
158901	3	411517	7	NULL	NULL	0	NULL	N-terminal polybasic domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	AKAP79/150 is targeted to dendritic spine plasma membranes by an N-terminal polybasic domain that binds phosphoinositide lipids , F-actin , and cadherin cell adhesion molecules .
	manualset3
158902	4	411517	7	NULL	NULL	0	NULL	phosphoinositide lipids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	AKAP79/150 is targeted to dendritic spine plasma membranes by an N-terminal polybasic domain that binds phosphoinositide lipids , F-actin , and cadherin cell adhesion molecules .
	manualset3
158903	5	411517	7	NULL	NULL	0	NULL	F-actin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	AKAP79/150 is targeted to dendritic spine plasma membranes by an N-terminal polybasic domain that binds phosphoinositide lipids , F-actin , and cadherin cell adhesion molecules .
	manualset3
158904	6	411517	7	NULL	NULL	0	NULL	cadherin cell adhesion molecules	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	AKAP79/150 is targeted to dendritic spine plasma membranes by an N-terminal polybasic domain that binds phosphoinositide lipids , F-actin , and cadherin cell adhesion molecules .
	manualset3
158905	1	411518	7	NULL	NULL	0	NULL	 phosphorylated PgDREB2A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The phosphorylated PgDREB2A did not bind to the DREs .
	manualset3
158906	2	411518	7	NULL	NULL	0	NULL	DREs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The phosphorylated PgDREB2A did not bind to the DREs .
	manualset3
158907	1	411519	7	NULL	NULL	0	NULL	phosphorylated analogs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The phosphorylated analogs are synthesized with protective tert-butyl groups that after assembly on thin polycrystalline gold films are removed in an acidic deprotection solution to form the corresponding phosphate self-assembled monolayers ( SAMs ) .
	manualset3
158908	2	411519	7	NULL	NULL	0	NULL	 protective tert-butyl groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The phosphorylated analogs are synthesized with protective tert-butyl groups that after assembly on thin polycrystalline gold films are removed in an acidic deprotection solution to form the corresponding phosphate self-assembled monolayers ( SAMs ) .
	manualset3
158909	3	411519	7	NULL	NULL	0	NULL	assembly	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The phosphorylated analogs are synthesized with protective tert-butyl groups that after assembly on thin polycrystalline gold films are removed in an acidic deprotection solution to form the corresponding phosphate self-assembled monolayers ( SAMs ) .
	manualset3
158910	4	411519	7	NULL	NULL	0	NULL	polycrystalline gold films	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The phosphorylated analogs are synthesized with protective tert-butyl groups that after assembly on thin polycrystalline gold films are removed in an acidic deprotection solution to form the corresponding phosphate self-assembled monolayers ( SAMs ) .
	manualset3
158911	5	411519	7	NULL	NULL	0	NULL	acidic deprotection solution 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The phosphorylated analogs are synthesized with protective tert-butyl groups that after assembly on thin polycrystalline gold films are removed in an acidic deprotection solution to form the corresponding phosphate self-assembled monolayers ( SAMs ) .
	manualset3
158912	6	411519	7	NULL	NULL	0	NULL	phosphate self-assembled monolayers ( SAMs )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The phosphorylated analogs are synthesized with protective tert-butyl groups that after assembly on thin polycrystalline gold films are removed in an acidic deprotection solution to form the corresponding phosphate self-assembled monolayers ( SAMs ) .
	manualset3
158913	1	411520	7	NULL	NULL	0	NULL	phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The phosphorylation is blocked by Ca2 + and CaM and reversed by the CaM-stimulated phosphatase ( calcineurin ) .
	manualset3
158914	2	411520	7	NULL	NULL	0	NULL	Ca2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The phosphorylation is blocked by Ca2 + and CaM and reversed by the CaM-stimulated phosphatase ( calcineurin ) .
	manualset3
158915	3	411520	7	NULL	NULL	0	NULL	CaM	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The phosphorylation is blocked by Ca2 + and CaM and reversed by the CaM-stimulated phosphatase ( calcineurin ) .
	manualset3
158916	4	411520	7	NULL	NULL	0	NULL	CaM-stimulated phosphatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The phosphorylation is blocked by Ca2 + and CaM and reversed by the CaM-stimulated phosphatase ( calcineurin ) .
	manualset3
158917	5	411520	7	NULL	NULL	0	NULL	calcineurin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The phosphorylation is blocked by Ca2 + and CaM and reversed by the CaM-stimulated phosphatase ( calcineurin ) .
	manualset3
158918	1	411521	7	NULL	NULL	0	NULL	phosphorylation status	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The phosphorylation status of PTS components reflects the availability of carbohydrates and the energy conditions of the cell .
	manualset3
158919	2	411521	7	NULL	NULL	0	NULL	PTS components	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The phosphorylation status of PTS components reflects the availability of carbohydrates and the energy conditions of the cell .
	manualset3
158920	3	411521	7	NULL	NULL	0	NULL	carbohydrates	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The phosphorylation status of PTS components reflects the availability of carbohydrates and the energy conditions of the cell .
	manualset3
158921	4	411521	7	NULL	NULL	0	NULL	energy conditions	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The phosphorylation status of PTS components reflects the availability of carbohydrates and the energy conditions of the cell .
	manualset3
158922	5	411521	7	NULL	NULL	0	NULL	cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The phosphorylation status of PTS components reflects the availability of carbohydrates and the energy conditions of the cell .
	manualset3
159052	6	411521	7	NULL	NULL	0	NULL	availability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The phosphorylation status of PTS components reflects the availability of carbohydrates and the energy conditions of the cell .
	manualset3
158923	1	411522	7	NULL	NULL	0	NULL	photodegradation process 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The photodegradation process was assayed by means of UV spectrophotometry and the reversed phase High-Performance Liquid Chromatography ( HPLC ) .
	manualset3
158924	2	411522	7	NULL	NULL	0	NULL	UV spectrophotometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The photodegradation process was assayed by means of UV spectrophotometry and the reversed phase High-Performance Liquid Chromatography ( HPLC ) .
	manualset3
158925	3	411522	7	NULL	NULL	0	NULL	reversed phase High-Performance Liquid Chromatography ( HPLC )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The photodegradation process was assayed by means of UV spectrophotometry and the reversed phase High-Performance Liquid Chromatography ( HPLC ) .
	manualset3
162359	4	411522	7	NULL	NULL	0	NULL	means	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The photodegradation process was assayed by means of UV spectrophotometry and the reversed phase High-Performance Liquid Chromatography ( HPLC ) .
	manualset3
158926	1	411523	7	NULL	NULL	0	NULL	photodynamic efficacy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The photodynamic efficacy of the DPcZn was drastically improved by the incorporation into the polymeric micelles , typically exhibiting more than two orders of magnitude higher photocytotoxicity compared with the free DPcZn at 60-min photoirradiation .
	manualset3
158927	2	411523	7	NULL	NULL	0	NULL	DPcZn	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The photodynamic efficacy of the DPcZn was drastically improved by the incorporation into the polymeric micelles , typically exhibiting more than two orders of magnitude higher photocytotoxicity compared with the free DPcZn at 60-min photoirradiation .
	manualset3
158928	3	411523	7	NULL	NULL	0	NULL	incorporation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The photodynamic efficacy of the DPcZn was drastically improved by the incorporation into the polymeric micelles , typically exhibiting more than two orders of magnitude higher photocytotoxicity compared with the free DPcZn at 60-min photoirradiation .
	manualset3
158929	4	411523	7	NULL	NULL	0	NULL	 polymeric micelles	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The photodynamic efficacy of the DPcZn was drastically improved by the incorporation into the polymeric micelles , typically exhibiting more than two orders of magnitude higher photocytotoxicity compared with the free DPcZn at 60-min photoirradiation .
	manualset3
158930	5	411523	7	NULL	NULL	0	NULL	two orders of magnitude 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The photodynamic efficacy of the DPcZn was drastically improved by the incorporation into the polymeric micelles , typically exhibiting more than two orders of magnitude higher photocytotoxicity compared with the free DPcZn at 60-min photoirradiation .
	manualset3
158931	6	411523	7	NULL	NULL	0	NULL	photocytotoxicity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The photodynamic efficacy of the DPcZn was drastically improved by the incorporation into the polymeric micelles , typically exhibiting more than two orders of magnitude higher photocytotoxicity compared with the free DPcZn at 60-min photoirradiation .
	manualset3
158932	7	411523	7	NULL	NULL	0	NULL	free DPcZn	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The photodynamic efficacy of the DPcZn was drastically improved by the incorporation into the polymeric micelles , typically exhibiting more than two orders of magnitude higher photocytotoxicity compared with the free DPcZn at 60-min photoirradiation .
	manualset3
158933	8	411523	7	NULL	NULL	0	NULL	60-min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The photodynamic efficacy of the DPcZn was drastically improved by the incorporation into the polymeric micelles , typically exhibiting more than two orders of magnitude higher photocytotoxicity compared with the free DPcZn at 60-min photoirradiation .
	manualset3
158934	9	411523	7	NULL	NULL	0	NULL	photoirradiation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The photodynamic efficacy of the DPcZn was drastically improved by the incorporation into the polymeric micelles , typically exhibiting more than two orders of magnitude higher photocytotoxicity compared with the free DPcZn at 60-min photoirradiation .
	manualset3
158935	1	411524	7	NULL	NULL	0	NULL	photographs	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The photographs observed by field-emission scanning electron microscopy ( FE-SEM ) show that a uniform titania mesoporous thin film with monodisperse TiO ( 2 ) spherical nanoparticles of ca .
	manualset3
158936	2	411524	7	NULL	NULL	0	NULL	field-emission scanning electron microscopy ( FE-SEM )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The photographs observed by field-emission scanning electron microscopy ( FE-SEM ) show that a uniform titania mesoporous thin film with monodisperse TiO ( 2 ) spherical nanoparticles of ca .
	manualset3
158937	3	411524	7	NULL	NULL	0	NULL	uniform titania mesoporous thin film 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The photographs observed by field-emission scanning electron microscopy ( FE-SEM ) show that a uniform titania mesoporous thin film with monodisperse TiO ( 2 ) spherical nanoparticles of ca .
	manualset3
158938	4	411524	7	NULL	NULL	0	NULL	monodisperse TiO ( 2 ) spherical nanoparticles of ca 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The photographs observed by field-emission scanning electron microscopy ( FE-SEM ) show that a uniform titania mesoporous thin film with monodisperse TiO ( 2 ) spherical nanoparticles of ca .
	manualset3
158939	1	411525	7	NULL	NULL	0	NULL	photon intensity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The photon intensity is measured by gating the channel of the spectrometer at FWHM/photo peak .
	manualset3
158940	2	411525	7	NULL	NULL	0	NULL	gating the channel	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The photon intensity is measured by gating the channel of the spectrometer at FWHM/photo peak .
	manualset3
158941	3	411525	7	NULL	NULL	0	NULL	spectrometer	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The photon intensity is measured by gating the channel of the spectrometer at FWHM/photo peak .
	manualset3
158942	4	411525	7	NULL	NULL	0	NULL	FWHM/photo peak	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The photon intensity is measured by gating the channel of the spectrometer at FWHM/photo peak .
	manualset3
158943	1	411526	7	NULL	NULL	0	NULL	phylogenetic hypotheses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The phylogenetic , ontogenetic and seasonal hypotheses on the annual periodicity of menarche were tested .
	manualset3
158944	2	411526	7	NULL	NULL	0	NULL	ontogenetic hypotheses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The phylogenetic , ontogenetic and seasonal hypotheses on the annual periodicity of menarche were tested .
	manualset3
158945	3	411526	7	NULL	NULL	0	NULL	seasonal hypotheses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The phylogenetic , ontogenetic and seasonal hypotheses on the annual periodicity of menarche were tested .
	manualset3
158946	4	411526	7	NULL	NULL	0	NULL	annual periodicity	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The phylogenetic , ontogenetic and seasonal hypotheses on the annual periodicity of menarche were tested .
	manualset3
158947	5	411526	7	NULL	NULL	0	NULL	menarche	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The phylogenetic , ontogenetic and seasonal hypotheses on the annual periodicity of menarche were tested .
	manualset3
158948	1	411527	7	NULL	NULL	0	NULL	AKR1B10 protein expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	AKR1B10 and AKR1B1 protein expression was inducible by bortezomib in HT-29 cells , but not detectable in SW-480 cells .
	manualset3
158949	2	411527	7	NULL	NULL	0	NULL	 AKR1B1 protein expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	AKR1B10 and AKR1B1 protein expression was inducible by bortezomib in HT-29 cells , but not detectable in SW-480 cells .
	manualset3
158950	3	411527	7	NULL	NULL	0	NULL	bortezomib	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	AKR1B10 and AKR1B1 protein expression was inducible by bortezomib in HT-29 cells , but not detectable in SW-480 cells .
	manualset3
158951	4	411527	7	NULL	NULL	0	NULL	HT-29 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	AKR1B10 and AKR1B1 protein expression was inducible by bortezomib in HT-29 cells , but not detectable in SW-480 cells .
	manualset3
158952	5	411527	7	NULL	NULL	0	NULL	SW-480 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	AKR1B10 and AKR1B1 protein expression was inducible by bortezomib in HT-29 cells , but not detectable in SW-480 cells .
	manualset3
158953	1	411528	7	NULL	NULL	NULL	NULL	phylogenetic tree	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The phylogenetic tree placed the ARbeaver-PV1 in a clade that included the Mupapillomavirus ( HPV1 and HPV63 ) and Kappapapillomavirus ( OcPV1 and SfPV1 ) genera .
	manualset3
158954	2	411528	7	NULL	NULL	NULL	NULL	ARbeaver-PV1	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The phylogenetic tree placed the ARbeaver-PV1 in a clade that included the Mupapillomavirus ( HPV1 and HPV63 ) and Kappapapillomavirus ( OcPV1 and SfPV1 ) genera .
	manualset3
158955	3	411528	7	NULL	NULL	NULL	NULL	clade	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The phylogenetic tree placed the ARbeaver-PV1 in a clade that included the Mupapillomavirus ( HPV1 and HPV63 ) and Kappapapillomavirus ( OcPV1 and SfPV1 ) genera .
	manualset3
158956	4	411528	7	NULL	NULL	0	NULL	Mupapillomavirus ( HPV1 and HPV63 ) genera	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The phylogenetic tree placed the ARbeaver-PV1 in a clade that included the Mupapillomavirus ( HPV1 and HPV63 ) and Kappapapillomavirus ( OcPV1 and SfPV1 ) genera .
	manualset3
158957	5	411528	7	NULL	NULL	0	NULL	Kappapapillomavirus ( OcPV1 and SfPV1 ) genera	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The phylogenetic tree placed the ARbeaver-PV1 in a clade that included the Mupapillomavirus ( HPV1 and HPV63 ) and Kappapapillomavirus ( OcPV1 and SfPV1 ) genera .
	manualset3
158958	1	411529	7	NULL	NULL	0	NULL	phylogeny	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The phylogeny and classification of parmelioid lichens has been a matter of debate for several decades .
	manualset3
158959	2	411529	7	NULL	NULL	NULL	NULL	classification 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The phylogeny and classification of parmelioid lichens has been a matter of debate for several decades .
	manualset3
158960	4	411529	7	NULL	NULL	NULL	NULL	debate	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The phylogeny and classification of parmelioid lichens has been a matter of debate for several decades .
	manualset3
158961	5	411529	7	NULL	NULL	NULL	NULL	several decades	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The phylogeny and classification of parmelioid lichens has been a matter of debate for several decades .
	manualset3
159053	3	411529	7	NULL	NULL	0	NULL	parmelioid lichens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The phylogeny and classification of parmelioid lichens has been a matter of debate for several decades .
	manualset3
158962	1	411530	7	NULL	NULL	NULL	NULL	physical properties	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The physical properties and molecular structure of Ligamentum nuchae elastin .
	manualset3
158963	2	411530	7	NULL	NULL	NULL	NULL	molecular structure 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The physical properties and molecular structure of Ligamentum nuchae elastin .
	manualset3
158964	3	411530	7	NULL	NULL	0	NULL	Ligamentum nuchae elastin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The physical properties and molecular structure of Ligamentum nuchae elastin .
	manualset3
158970	1	411531	7	NULL	NULL	0	NULL	physical stability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The physical stability of polyelectrolyte nanocomplexes composed of trimethyl chitosan ( TMC ) and hyaluronic acid ( HA ) is limited in physiological conditions .
	manualset3
158971	2	411531	7	NULL	NULL	0	NULL	polyelectrolyte nanocomplexes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The physical stability of polyelectrolyte nanocomplexes composed of trimethyl chitosan ( TMC ) and hyaluronic acid ( HA ) is limited in physiological conditions .
	manualset3
158972	3	411531	7	NULL	NULL	0	NULL	trimethyl chitosan ( TMC ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The physical stability of polyelectrolyte nanocomplexes composed of trimethyl chitosan ( TMC ) and hyaluronic acid ( HA ) is limited in physiological conditions .
	manualset3
158973	4	411531	7	NULL	NULL	0	NULL	hyaluronic acid ( HA ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The physical stability of polyelectrolyte nanocomplexes composed of trimethyl chitosan ( TMC ) and hyaluronic acid ( HA ) is limited in physiological conditions .
	manualset3
158974	5	411531	7	NULL	NULL	0	NULL	physiological conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The physical stability of polyelectrolyte nanocomplexes composed of trimethyl chitosan ( TMC ) and hyaluronic acid ( HA ) is limited in physiological conditions .
	manualset3
158965	1	411532	7	NULL	NULL	NULL	NULL	physicochemical properties	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The physicochemical properties of a model medium consisting of two substances , sodium sulfite and albumin , were studied .
	manualset3
158966	2	411532	7	NULL	NULL	NULL	NULL	sodium sulfite	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The physicochemical properties of a model medium consisting of two substances , sodium sulfite and albumin , were studied .
	manualset3
158967	3	411532	7	NULL	NULL	0	NULL	two substances	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The physicochemical properties of a model medium consisting of two substances , sodium sulfite and albumin , were studied .
	manualset3
158968	4	411532	7	NULL	NULL	0	NULL	albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The physicochemical properties of a model medium consisting of two substances , sodium sulfite and albumin , were studied .
	manualset3
158969	5	411532	7	NULL	NULL	0	NULL	model medium	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The physicochemical properties of a model medium consisting of two substances , sodium sulfite and albumin , were studied .
	manualset3
158975	1	411533	7	NULL	NULL	0	NULL	physiologic significance	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The physiologic significance of delayed DAG accumulation was investigated using the cell-permeable DAG analog , dioctanoylglycerol ( diC8 ) .
	manualset3
158976	2	411533	7	NULL	NULL	0	NULL	delayed DAG accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The physiologic significance of delayed DAG accumulation was investigated using the cell-permeable DAG analog , dioctanoylglycerol ( diC8 ) .
	manualset3
158977	3	411533	7	NULL	NULL	0	NULL	cell-permeable DAG analog 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The physiologic significance of delayed DAG accumulation was investigated using the cell-permeable DAG analog , dioctanoylglycerol ( diC8 ) .
	manualset3
158978	4	411533	7	NULL	NULL	0	NULL	dioctanoylglycerol ( diC8 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The physiologic significance of delayed DAG accumulation was investigated using the cell-permeable DAG analog , dioctanoylglycerol ( diC8 ) .
	manualset3
158979	1	411534	7	NULL	NULL	NULL	NULL	physiological properties 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The physiological properties of the cells in the suprageniculate nucleus and in the AES/insular cortex exhibited striking similarities in a series of aspects : ( a ) The frequencies of occurrence of uni - , bi - and trimodal cells were similar .
	manualset3
158980	2	411534	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The physiological properties of the cells in the suprageniculate nucleus and in the AES/insular cortex exhibited striking similarities in a series of aspects : ( a ) The frequencies of occurrence of uni - , bi - and trimodal cells were similar .
	manualset3
158981	3	411534	7	NULL	NULL	0	NULL	suprageniculate nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The physiological properties of the cells in the suprageniculate nucleus and in the AES/insular cortex exhibited striking similarities in a series of aspects : ( a ) The frequencies of occurrence of uni - , bi - and trimodal cells were similar .
	manualset3
158982	4	411534	7	NULL	NULL	NULL	NULL	AES/insular cortex	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The physiological properties of the cells in the suprageniculate nucleus and in the AES/insular cortex exhibited striking similarities in a series of aspects : ( a ) The frequencies of occurrence of uni - , bi - and trimodal cells were similar .
	manualset3
158983	5	411534	7	NULL	NULL	NULL	NULL	aspects 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The physiological properties of the cells in the suprageniculate nucleus and in the AES/insular cortex exhibited striking similarities in a series of aspects : ( a ) The frequencies of occurrence of uni - , bi - and trimodal cells were similar .
	manualset3
158984	6	411534	7	NULL	NULL	0	NULL	frequencies 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The physiological properties of the cells in the suprageniculate nucleus and in the AES/insular cortex exhibited striking similarities in a series of aspects : ( a ) The frequencies of occurrence of uni - , bi - and trimodal cells were similar .
	manualset3
158985	7	411534	7	NULL	NULL	NULL	NULL	unimodal cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The physiological properties of the cells in the suprageniculate nucleus and in the AES/insular cortex exhibited striking similarities in a series of aspects : ( a ) The frequencies of occurrence of uni - , bi - and trimodal cells were similar .
	manualset3
158986	8	411534	7	NULL	NULL	0	NULL	bimodal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The physiological properties of the cells in the suprageniculate nucleus and in the AES/insular cortex exhibited striking similarities in a series of aspects : ( a ) The frequencies of occurrence of uni - , bi - and trimodal cells were similar .
	manualset3
158987	9	411534	7	NULL	NULL	0	NULL	trimodal cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The physiological properties of the cells in the suprageniculate nucleus and in the AES/insular cortex exhibited striking similarities in a series of aspects : ( a ) The frequencies of occurrence of uni - , bi - and trimodal cells were similar .
	manualset3
162695	10	411534	7	NULL	NULL	0	NULL	similarities	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The physiological properties of the cells in the suprageniculate nucleus and in the AES/insular cortex exhibited striking similarities in a series of aspects : ( a ) The frequencies of occurrence of uni - , bi - and trimodal cells were similar .
	manualset3
158988	1	411535	7	NULL	NULL	0	NULL	ALA	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	ALA prevented the strong expression of heme oxygenase by As ( 3 + ) exposure ( from 35 - to 5-times of control cells ) , which correlated with the reduction of Nrf2 observed in As ( 3 + ) group .
	manualset3
158989	2	411535	7	NULL	NULL	NULL	NULL	strong expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ALA prevented the strong expression of heme oxygenase by As ( 3 + ) exposure ( from 35 - to 5-times of control cells ) , which correlated with the reduction of Nrf2 observed in As ( 3 + ) group .
	manualset3
158990	3	411535	7	NULL	NULL	0	NULL	heme oxygenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	ALA prevented the strong expression of heme oxygenase by As ( 3 + ) exposure ( from 35 - to 5-times of control cells ) , which correlated with the reduction of Nrf2 observed in As ( 3 + ) group .
	manualset3
158991	4	411535	7	NULL	NULL	NULL	NULL	As ( 3 + ) exposure	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ALA prevented the strong expression of heme oxygenase by As ( 3 + ) exposure ( from 35 - to 5-times of control cells ) , which correlated with the reduction of Nrf2 observed in As ( 3 + ) group .
	manualset3
158992	5	411535	7	NULL	NULL	NULL	NULL	35 - to 5-times 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ALA prevented the strong expression of heme oxygenase by As ( 3 + ) exposure ( from 35 - to 5-times of control cells ) , which correlated with the reduction of Nrf2 observed in As ( 3 + ) group .
	manualset3
158993	7	411535	7	NULL	NULL	NULL	NULL	reduction	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ALA prevented the strong expression of heme oxygenase by As ( 3 + ) exposure ( from 35 - to 5-times of control cells ) , which correlated with the reduction of Nrf2 observed in As ( 3 + ) group .
	manualset3
158994	9	411535	7	NULL	NULL	NULL	NULL	As ( 3 + ) group	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ALA prevented the strong expression of heme oxygenase by As ( 3 + ) exposure ( from 35 - to 5-times of control cells ) , which correlated with the reduction of Nrf2 observed in As ( 3 + ) group .
	manualset3
158995	6	411535	7	NULL	NULL	0	NULL	control cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	ALA prevented the strong expression of heme oxygenase by As ( 3 + ) exposure ( from 35 - to 5-times of control cells ) , which correlated with the reduction of Nrf2 observed in As ( 3 + ) group .
	manualset3
160306	8	411535	7	NULL	NULL	0	NULL	Nrf2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	ALA prevented the strong expression of heme oxygenase by As ( 3 + ) exposure ( from 35 - to 5-times of control cells ) , which correlated with the reduction of Nrf2 observed in As ( 3 + ) group .
	manualset3
158996	1	411536	7	NULL	NULL	0	NULL	physiological regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The physiological regulation of melanocyte proliferation and differentiation is not yet fully defined and this study summarises several separate lines of evidence which suggest that , in vivo , some of the signals required for melanocyte proliferation and differentiation may derive from extracellular matrix ( ECM ) proteins adjacent to these cells .
	manualset3
158997	2	411536	7	NULL	NULL	NULL	NULL	melanocyte proliferation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The physiological regulation of melanocyte proliferation and differentiation is not yet fully defined and this study summarises several separate lines of evidence which suggest that , in vivo , some of the signals required for melanocyte proliferation and differentiation may derive from extracellular matrix ( ECM ) proteins adjacent to these cells .
	manualset3
158998	3	411536	7	NULL	NULL	NULL	NULL	melanocyte differentiation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The physiological regulation of melanocyte proliferation and differentiation is not yet fully defined and this study summarises several separate lines of evidence which suggest that , in vivo , some of the signals required for melanocyte proliferation and differentiation may derive from extracellular matrix ( ECM ) proteins adjacent to these cells .
	manualset3
158999	4	411536	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The physiological regulation of melanocyte proliferation and differentiation is not yet fully defined and this study summarises several separate lines of evidence which suggest that , in vivo , some of the signals required for melanocyte proliferation and differentiation may derive from extracellular matrix ( ECM ) proteins adjacent to these cells .
	manualset3
159000	5	411536	7	NULL	NULL	0	NULL	lines of evidence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The physiological regulation of melanocyte proliferation and differentiation is not yet fully defined and this study summarises several separate lines of evidence which suggest that , in vivo , some of the signals required for melanocyte proliferation and differentiation may derive from extracellular matrix ( ECM ) proteins adjacent to these cells .
	manualset3
159002	7	411536	7	NULL	NULL	0	NULL	signals 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The physiological regulation of melanocyte proliferation and differentiation is not yet fully defined and this study summarises several separate lines of evidence which suggest that , in vivo , some of the signals required for melanocyte proliferation and differentiation may derive from extracellular matrix ( ECM ) proteins adjacent to these cells .
	manualset3
159003	8	411536	7	NULL	NULL	NULL	NULL	melanocyte proliferation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The physiological regulation of melanocyte proliferation and differentiation is not yet fully defined and this study summarises several separate lines of evidence which suggest that , in vivo , some of the signals required for melanocyte proliferation and differentiation may derive from extracellular matrix ( ECM ) proteins adjacent to these cells .
	manualset3
159004	9	411536	7	NULL	NULL	NULL	NULL	melanocyte differentiation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The physiological regulation of melanocyte proliferation and differentiation is not yet fully defined and this study summarises several separate lines of evidence which suggest that , in vivo , some of the signals required for melanocyte proliferation and differentiation may derive from extracellular matrix ( ECM ) proteins adjacent to these cells .
	manualset3
159005	10	411536	7	NULL	NULL	NULL	NULL	extracellular matrix ( ECM ) proteins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The physiological regulation of melanocyte proliferation and differentiation is not yet fully defined and this study summarises several separate lines of evidence which suggest that , in vivo , some of the signals required for melanocyte proliferation and differentiation may derive from extracellular matrix ( ECM ) proteins adjacent to these cells .
	manualset3
159006	11	411536	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The physiological regulation of melanocyte proliferation and differentiation is not yet fully defined and this study summarises several separate lines of evidence which suggest that , in vivo , some of the signals required for melanocyte proliferation and differentiation may derive from extracellular matrix ( ECM ) proteins adjacent to these cells .
	manualset3
159007	1	411537	7	NULL	NULL	0	NULL	physiological relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The physiological relationship between typhus rickettsiae and their host cells .
	manualset3
159008	2	411537	7	NULL	NULL	0	NULL	typhus rickettsiae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The physiological relationship between typhus rickettsiae and their host cells .
	manualset3
159009	3	411537	7	NULL	NULL	0	NULL	host cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The physiological relationship between typhus rickettsiae and their host cells .
	manualset3
159010	1	411538	7	NULL	NULL	0	NULL	place	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The place of autonomy in bioethics .
	manualset3
159011	2	411538	7	NULL	NULL	0	NULL	autonomy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The place of autonomy in bioethics .
	manualset3
159012	3	411538	7	NULL	NULL	0	NULL	bioethics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The place of autonomy in bioethics .
	manualset3
159013	1	411539	7	NULL	NULL	NULL	NULL	place	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The place of tenecteplase in management of STEMI .
	manualset3
159014	2	411539	7	NULL	NULL	0	NULL	tenecteplase	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The place of tenecteplase in management of STEMI .
	manualset3
159015	3	411539	7	NULL	NULL	0	NULL	STEMI	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The place of tenecteplase in management of STEMI .
	manualset3
162696	4	411539	7	NULL	NULL	0	NULL	management 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The place of tenecteplase in management of STEMI .
	manualset3
159016	1	411540	7	NULL	NULL	0	NULL	planar benzimidazole ring systems	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The planar benzimidazole ring systems are oriented with respect to the phen-yl/fluoro-benzene rings at dihedral angles of 31.10 ( 4 ) / 45.17 ( 5 ) and 45.52 ( 5 ) / 68.63 ( 5 ) , respectively , for the two mol-ecules .
	manualset3
159017	2	411540	7	NULL	NULL	0	NULL	phen-yl/fluoro-benzene rings 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The planar benzimidazole ring systems are oriented with respect to the phen-yl/fluoro-benzene rings at dihedral angles of 31.10 ( 4 ) / 45.17 ( 5 ) and 45.52 ( 5 ) / 68.63 ( 5 ) , respectively , for the two mol-ecules .
	manualset3
159018	3	411540	7	NULL	NULL	0	NULL	dihedral angles	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The planar benzimidazole ring systems are oriented with respect to the phen-yl/fluoro-benzene rings at dihedral angles of 31.10 ( 4 ) / 45.17 ( 5 ) and 45.52 ( 5 ) / 68.63 ( 5 ) , respectively , for the two mol-ecules .
	manualset3
159019	4	411540	7	NULL	NULL	0	NULL	31.10 ( 4 ) / 45.17 ( 5 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The planar benzimidazole ring systems are oriented with respect to the phen-yl/fluoro-benzene rings at dihedral angles of 31.10 ( 4 ) / 45.17 ( 5 ) and 45.52 ( 5 ) / 68.63 ( 5 ) , respectively , for the two mol-ecules .
	manualset3
159020	5	411540	7	NULL	NULL	0	NULL	45.52 ( 5 ) / 68.63 ( 5 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The planar benzimidazole ring systems are oriented with respect to the phen-yl/fluoro-benzene rings at dihedral angles of 31.10 ( 4 ) / 45.17 ( 5 ) and 45.52 ( 5 ) / 68.63 ( 5 ) , respectively , for the two mol-ecules .
	manualset3
159021	6	411540	7	NULL	NULL	0	NULL	two mol-ecules 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The planar benzimidazole ring systems are oriented with respect to the phen-yl/fluoro-benzene rings at dihedral angles of 31.10 ( 4 ) / 45.17 ( 5 ) and 45.52 ( 5 ) / 68.63 ( 5 ) , respectively , for the two mol-ecules .
	manualset3
159022	1	411541	7	NULL	NULL	0	NULL	plant	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The plant is in a municipality close to Monterrey , which is Mexico 's third most populous and second most industrialized city .
	manualset3
159023	2	411541	7	NULL	NULL	0	NULL	municipality	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The plant is in a municipality close to Monterrey , which is Mexico 's third most populous and second most industrialized city .
	manualset3
159024	3	411541	7	NULL	NULL	0	NULL	Monterrey	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The plant is in a municipality close to Monterrey , which is Mexico 's third most populous and second most industrialized city .
	manualset3
159025	4	411541	7	NULL	NULL	0	NULL	Mexico	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The plant is in a municipality close to Monterrey , which is Mexico 's third most populous and second most industrialized city .
	manualset3
159026	5	411541	7	NULL	NULL	NULL	NULL	industrialized city	GeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The plant is in a municipality close to Monterrey , which is Mexico 's third most populous and second most industrialized city .
	manualset3
159027	1	411542	7	NULL	NULL	0	NULL	plaques	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The plaques were mineralised with a urea-based , calcium-phosphate-monofluorophosphate-urea ( CPMU ) mineralising solution .
	manualset3
159029	2	411542	7	NULL	NULL	NULL	NULL	urea-based,calcium-phosphate-monofluorophosphate-urea ( CPMU ) mineralising solution	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The plaques were mineralised with a urea-based , calcium-phosphate-monofluorophosphate-urea ( CPMU ) mineralising solution .
	manualset3
159030	1	411543	7	NULL	NULL	0	NULL	plasma HDL-cholesterol concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma HDL-cholesterol concentration and ratio of HDL to total cholesterol were significantly higher in 1 and 2 groups than in control group .
	manualset3
159031	2	411543	7	NULL	NULL	0	NULL	ratio of HDL to total cholesterol	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma HDL-cholesterol concentration and ratio of HDL to total cholesterol were significantly higher in 1 and 2 groups than in control group .
	manualset3
159032	3	411543	7	NULL	NULL	0	NULL	1 and 2 groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma HDL-cholesterol concentration and ratio of HDL to total cholesterol were significantly higher in 1 and 2 groups than in control group .
	manualset3
159033	4	411543	7	NULL	NULL	0	NULL	control group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma HDL-cholesterol concentration and ratio of HDL to total cholesterol were significantly higher in 1 and 2 groups than in control group .
	manualset3
159034	1	411544	7	NULL	NULL	0	NULL	ALBERT FISCHER	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	ALBERT FISCHER , 23/7 1891-31/7 1956 .
	manualset3
159035	2	411544	7	NULL	NULL	NULL	NULL	23/7 1891-31/7 1956	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ALBERT FISCHER , 23/7 1891-31/7 1956 .
	manualset3
159045	1	411545	7	NULL	NULL	0	NULL	 plasma NE levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma NE and E levels were both increased in OMI and DCM , particularly in the coronary sinus , as compared with those in 16 control subjects ( Control ) .
	manualset3
159046	2	411545	7	NULL	NULL	0	NULL	E levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma NE and E levels were both increased in OMI and DCM , particularly in the coronary sinus , as compared with those in 16 control subjects ( Control ) .
	manualset3
159047	3	411545	7	NULL	NULL	0	NULL	OMI	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma NE and E levels were both increased in OMI and DCM , particularly in the coronary sinus , as compared with those in 16 control subjects ( Control ) .
	manualset3
159048	4	411545	7	NULL	NULL	0	NULL	DCM 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma NE and E levels were both increased in OMI and DCM , particularly in the coronary sinus , as compared with those in 16 control subjects ( Control ) .
	manualset3
159049	5	411545	7	NULL	NULL	0	NULL	coronary sinus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma NE and E levels were both increased in OMI and DCM , particularly in the coronary sinus , as compared with those in 16 control subjects ( Control ) .
	manualset3
159050	6	411545	7	NULL	NULL	0	NULL	16 control subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma NE and E levels were both increased in OMI and DCM , particularly in the coronary sinus , as compared with those in 16 control subjects ( Control ) .
	manualset3
159051	7	411545	7	NULL	NULL	0	NULL	Control 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma NE and E levels were both increased in OMI and DCM , particularly in the coronary sinus , as compared with those in 16 control subjects ( Control ) .
	manualset3
159057	1	411546	7	NULL	NULL	0	NULL	 plasma TG pool	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma TG pool was 33-40 % larger with beef tallow than with corn , olive or coconut oil feeding ( p less than 0.05 ) , and 20 % larger with beef tallow than with butterfat feeding .
	manualset3
159058	2	411546	7	NULL	NULL	0	NULL	33-40 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma TG pool was 33-40 % larger with beef tallow than with corn , olive or coconut oil feeding ( p less than 0.05 ) , and 20 % larger with beef tallow than with butterfat feeding .
	manualset3
159059	3	411546	7	NULL	NULL	0	NULL	 beef tallow	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma TG pool was 33-40 % larger with beef tallow than with corn , olive or coconut oil feeding ( p less than 0.05 ) , and 20 % larger with beef tallow than with butterfat feeding .
	manualset3
159060	4	411546	7	NULL	NULL	0	NULL	corn oil feeding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma TG pool was 33-40 % larger with beef tallow than with corn , olive or coconut oil feeding ( p less than 0.05 ) , and 20 % larger with beef tallow than with butterfat feeding .
	manualset3
159061	5	411546	7	NULL	NULL	0	NULL	 olive oil feeding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma TG pool was 33-40 % larger with beef tallow than with corn , olive or coconut oil feeding ( p less than 0.05 ) , and 20 % larger with beef tallow than with butterfat feeding .
	manualset3
159062	6	411546	7	NULL	NULL	0	NULL	coconut oil feeding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma TG pool was 33-40 % larger with beef tallow than with corn , olive or coconut oil feeding ( p less than 0.05 ) , and 20 % larger with beef tallow than with butterfat feeding .
	manualset3
159063	7	411546	7	NULL	NULL	0	NULL	p less than 0.05 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma TG pool was 33-40 % larger with beef tallow than with corn , olive or coconut oil feeding ( p less than 0.05 ) , and 20 % larger with beef tallow than with butterfat feeding .
	manualset3
159064	8	411546	7	NULL	NULL	0	NULL	20 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma TG pool was 33-40 % larger with beef tallow than with corn , olive or coconut oil feeding ( p less than 0.05 ) , and 20 % larger with beef tallow than with butterfat feeding .
	manualset3
159065	9	411546	7	NULL	NULL	0	NULL	beef tallow	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma TG pool was 33-40 % larger with beef tallow than with corn , olive or coconut oil feeding ( p less than 0.05 ) , and 20 % larger with beef tallow than with butterfat feeding .
	manualset3
159066	10	411546	7	NULL	NULL	0	NULL	butterfat feeding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma TG pool was 33-40 % larger with beef tallow than with corn , olive or coconut oil feeding ( p less than 0.05 ) , and 20 % larger with beef tallow than with butterfat feeding .
	manualset3
159067	1	411547	7	NULL	NULL	0	NULL	plasma concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma concentrations of glucose , insulin , epinephrine , norepinephrine and cortisol were measured in 18 women before , during and after abdominal hysterectomy .
	manualset3
159068	2	411547	7	NULL	NULL	NULL	NULL	glucose	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The plasma concentrations of glucose , insulin , epinephrine , norepinephrine and cortisol were measured in 18 women before , during and after abdominal hysterectomy .
	manualset3
159069	3	411547	7	NULL	NULL	0	NULL	insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma concentrations of glucose , insulin , epinephrine , norepinephrine and cortisol were measured in 18 women before , during and after abdominal hysterectomy .
	manualset3
159070	4	411547	7	NULL	NULL	0	NULL	epinephrine	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma concentrations of glucose , insulin , epinephrine , norepinephrine and cortisol were measured in 18 women before , during and after abdominal hysterectomy .
	manualset3
159071	5	411547	7	NULL	NULL	0	NULL	norepinephrine 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma concentrations of glucose , insulin , epinephrine , norepinephrine and cortisol were measured in 18 women before , during and after abdominal hysterectomy .
	manualset3
159072	6	411547	7	NULL	NULL	0	NULL	cortisol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma concentrations of glucose , insulin , epinephrine , norepinephrine and cortisol were measured in 18 women before , during and after abdominal hysterectomy .
	manualset3
159073	7	411547	7	NULL	NULL	0	NULL	18 women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma concentrations of glucose , insulin , epinephrine , norepinephrine and cortisol were measured in 18 women before , during and after abdominal hysterectomy .
	manualset3
159074	8	411547	7	NULL	NULL	0	NULL	abdominal hysterectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma concentrations of glucose , insulin , epinephrine , norepinephrine and cortisol were measured in 18 women before , during and after abdominal hysterectomy .
	manualset3
159075	1	411548	7	NULL	NULL	0	NULL	 plasma glibenclamide concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma glibenclamide concentration was 158 + / -29 micro M , whereas that in the tubular fluid entering the LOH was below detectable limits ( 10 micro M ) .
	manualset3
159076	2	411548	7	NULL	NULL	0	NULL	158 + / -29 micro M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma glibenclamide concentration was 158 + / -29 micro M , whereas that in the tubular fluid entering the LOH was below detectable limits ( 10 micro M ) .
	manualset3
159077	3	411548	7	NULL	NULL	0	NULL	 tubular fluid	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma glibenclamide concentration was 158 + / -29 micro M , whereas that in the tubular fluid entering the LOH was below detectable limits ( 10 micro M ) .
	manualset3
159078	4	411548	7	NULL	NULL	0	NULL	LOH	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma glibenclamide concentration was 158 + / -29 micro M , whereas that in the tubular fluid entering the LOH was below detectable limits ( 10 micro M ) .
	manualset3
159079	5	411548	7	NULL	NULL	0	NULL	detectable limits 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma glibenclamide concentration was 158 + / -29 micro M , whereas that in the tubular fluid entering the LOH was below detectable limits ( 10 micro M ) .
	manualset3
159080	6	411548	7	NULL	NULL	0	NULL	10 micro M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma glibenclamide concentration was 158 + / -29 micro M , whereas that in the tubular fluid entering the LOH was below detectable limits ( 10 micro M ) .
	manualset3
159081	1	411549	7	NULL	NULL	0	NULL	 plasma membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma membrane H + - ATPase couples ATP hydrolysis to proton transport , thereby establishing the driving force for solute transport across the plasma membrane .
	manualset3
159082	2	411549	7	NULL	NULL	0	NULL	H + - ATPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma membrane H + - ATPase couples ATP hydrolysis to proton transport , thereby establishing the driving force for solute transport across the plasma membrane .
	manualset3
159083	3	411549	7	NULL	NULL	0	NULL	ATP hydrolysis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma membrane H + - ATPase couples ATP hydrolysis to proton transport , thereby establishing the driving force for solute transport across the plasma membrane .
	manualset3
159084	4	411549	7	NULL	NULL	0	NULL	proton transport	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma membrane H + - ATPase couples ATP hydrolysis to proton transport , thereby establishing the driving force for solute transport across the plasma membrane .
	manualset3
159085	5	411549	7	NULL	NULL	0	NULL	driving force	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma membrane H + - ATPase couples ATP hydrolysis to proton transport , thereby establishing the driving force for solute transport across the plasma membrane .
	manualset3
159086	6	411549	7	NULL	NULL	0	NULL	solute transport	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma membrane H + - ATPase couples ATP hydrolysis to proton transport , thereby establishing the driving force for solute transport across the plasma membrane .
	manualset3
159087	7	411549	7	NULL	NULL	0	NULL	plasma membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma membrane H + - ATPase couples ATP hydrolysis to proton transport , thereby establishing the driving force for solute transport across the plasma membrane .
	manualset3
159088	1	411550	7	NULL	NULL	0	NULL	plasma membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma membrane monoamine transporters terminate neurotransmission by removing dopamine , norepinephrine , or serotonin from the synaptic cleft between neurons .
	manualset3
159089	2	411550	7	NULL	NULL	0	NULL	monoamine transporters	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma membrane monoamine transporters terminate neurotransmission by removing dopamine , norepinephrine , or serotonin from the synaptic cleft between neurons .
	manualset3
159090	3	411550	7	NULL	NULL	NULL	NULL	terminate	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The plasma membrane monoamine transporters terminate neurotransmission by removing dopamine , norepinephrine , or serotonin from the synaptic cleft between neurons .
	manualset3
159091	4	411550	7	NULL	NULL	0	NULL	neurotransmission	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma membrane monoamine transporters terminate neurotransmission by removing dopamine , norepinephrine , or serotonin from the synaptic cleft between neurons .
	manualset3
159092	5	411550	7	NULL	NULL	0	NULL	dopamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma membrane monoamine transporters terminate neurotransmission by removing dopamine , norepinephrine , or serotonin from the synaptic cleft between neurons .
	manualset3
159093	6	411550	7	NULL	NULL	0	NULL	norepinephrine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma membrane monoamine transporters terminate neurotransmission by removing dopamine , norepinephrine , or serotonin from the synaptic cleft between neurons .
	manualset3
159094	7	411550	7	NULL	NULL	0	NULL	serotonin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma membrane monoamine transporters terminate neurotransmission by removing dopamine , norepinephrine , or serotonin from the synaptic cleft between neurons .
	manualset3
159095	8	411550	7	NULL	NULL	0	NULL	synaptic cleft	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma membrane monoamine transporters terminate neurotransmission by removing dopamine , norepinephrine , or serotonin from the synaptic cleft between neurons .
	manualset3
159096	9	411550	7	NULL	NULL	NULL	NULL	neurons	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The plasma membrane monoamine transporters terminate neurotransmission by removing dopamine , norepinephrine , or serotonin from the synaptic cleft between neurons .
	manualset3
159097	1	411551	7	NULL	NULL	0	NULL	plasma parameters 	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma parameters and ultrastructural morphology changes were increased markedly 24hr after the treatment of rats with CER .
	manualset3
159098	2	411551	7	NULL	NULL	0	NULL	ultrastructural morphology changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma parameters and ultrastructural morphology changes were increased markedly 24hr after the treatment of rats with CER .
	manualset3
159099	3	411551	7	NULL	NULL	0	NULL	24hr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma parameters and ultrastructural morphology changes were increased markedly 24hr after the treatment of rats with CER .
	manualset3
159100	4	411551	7	NULL	NULL	0	NULL	treatment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma parameters and ultrastructural morphology changes were increased markedly 24hr after the treatment of rats with CER .
	manualset3
159101	5	411551	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma parameters and ultrastructural morphology changes were increased markedly 24hr after the treatment of rats with CER .
	manualset3
159102	6	411551	7	NULL	NULL	0	NULL	CER	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma parameters and ultrastructural morphology changes were increased markedly 24hr after the treatment of rats with CER .
	manualset3
159103	1	411552	7	NULL	NULL	0	NULL	plasma potential	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma potential increased with increasing gas pressure .
	manualset3
159104	2	411552	7	NULL	NULL	0	NULL	 increasing gas pressure 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma potential increased with increasing gas pressure .
	manualset3
159105	1	411553	7	NULL	NULL	0	NULL	Clinical presentations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical presentations of aneurysms and dissections of the aorta ) .
	manualset3
159106	2	411553	7	NULL	NULL	0	NULL	aneurysms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical presentations of aneurysms and dissections of the aorta ) .
	manualset3
159107	3	411553	7	NULL	NULL	NULL	NULL	dissections 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Clinical presentations of aneurysms and dissections of the aorta ) .
	manualset3
160309	4	411553	7	NULL	NULL	0	NULL	aorta	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical presentations of aneurysms and dissections of the aorta ) .
	manualset3
159108	1	411554	7	NULL	NULL	0	NULL	ALFRED	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	ALFRED ( http : //alfred.med.yale.edu ) is a free , web accessible , curated compilation of allele frequency data on DNA sequence polymorphisms in anthropologically defined human populations .
	manualset3
159109	2	411554	7	NULL	NULL	NULL	NULL	http : //alfred.med.yale.edu	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ALFRED ( http : //alfred.med.yale.edu ) is a free , web accessible , curated compilation of allele frequency data on DNA sequence polymorphisms in anthropologically defined human populations .
	manualset3
159110	3	411554	7	NULL	NULL	0	NULL	free	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	ALFRED ( http : //alfred.med.yale.edu ) is a free , web accessible , curated compilation of allele frequency data on DNA sequence polymorphisms in anthropologically defined human populations .
	manualset3
159111	4	411554	7	NULL	NULL	0	NULL	web accessible	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	ALFRED ( http : //alfred.med.yale.edu ) is a free , web accessible , curated compilation of allele frequency data on DNA sequence polymorphisms in anthropologically defined human populations .
	manualset3
159112	5	411554	7	NULL	NULL	0	NULL	curated compilation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	ALFRED ( http : //alfred.med.yale.edu ) is a free , web accessible , curated compilation of allele frequency data on DNA sequence polymorphisms in anthropologically defined human populations .
	manualset3
159113	6	411554	7	NULL	NULL	0	NULL	allele frequency data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	ALFRED ( http : //alfred.med.yale.edu ) is a free , web accessible , curated compilation of allele frequency data on DNA sequence polymorphisms in anthropologically defined human populations .
	manualset3
159114	7	411554	7	NULL	NULL	0	NULL	DNA sequence polymorphisms	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	ALFRED ( http : //alfred.med.yale.edu ) is a free , web accessible , curated compilation of allele frequency data on DNA sequence polymorphisms in anthropologically defined human populations .
	manualset3
159115	8	411554	7	NULL	NULL	0	NULL	human populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	ALFRED ( http : //alfred.med.yale.edu ) is a free , web accessible , curated compilation of allele frequency data on DNA sequence polymorphisms in anthropologically defined human populations .
	manualset3
159116	1	411555	7	NULL	NULL	NULL	NULL	plasma protein binding 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The plasma protein binding of diphenylhydantoin sodium was determined in 26 patients who had been taking diphenylhydantoin regularly for more than two weeks .
	manualset3
159117	2	411555	7	NULL	NULL	0	NULL	diphenylhydantoin sodium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma protein binding of diphenylhydantoin sodium was determined in 26 patients who had been taking diphenylhydantoin regularly for more than two weeks .
	manualset3
159118	3	411555	7	NULL	NULL	0	NULL	26 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma protein binding of diphenylhydantoin sodium was determined in 26 patients who had been taking diphenylhydantoin regularly for more than two weeks .
	manualset3
159119	4	411555	7	NULL	NULL	0	NULL	diphenylhydantoin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma protein binding of diphenylhydantoin sodium was determined in 26 patients who had been taking diphenylhydantoin regularly for more than two weeks .
	manualset3
159121	6	411555	7	NULL	NULL	0	NULL	two weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasma protein binding of diphenylhydantoin sodium was determined in 26 patients who had been taking diphenylhydantoin regularly for more than two weeks .
	manualset3
159122	1	411556	7	NULL	NULL	0	NULL	plasmacytoid dendritic cells ( pDCs )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasmacytoid dendritic cells ( pDCs ) express a high level of Toll-like receptor 9 ( TLR-9 ) , which recognizes viral DNA .
	manualset3
159123	2	411556	7	NULL	NULL	0	NULL	high level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasmacytoid dendritic cells ( pDCs ) express a high level of Toll-like receptor 9 ( TLR-9 ) , which recognizes viral DNA .
	manualset3
159124	3	411556	7	NULL	NULL	0	NULL	Toll-like receptor 9 ( TLR-9 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasmacytoid dendritic cells ( pDCs ) express a high level of Toll-like receptor 9 ( TLR-9 ) , which recognizes viral DNA .
	manualset3
159125	4	411556	7	NULL	NULL	0	NULL	viral DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasmacytoid dendritic cells ( pDCs ) express a high level of Toll-like receptor 9 ( TLR-9 ) , which recognizes viral DNA .
	manualset3
159126	1	411557	7	NULL	NULL	0	NULL	plasmid pMAL-p2x-mHD-5	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasmid pMAL-p2x-mHD-5 was transferred into engineered strain BL21 ( DE3 ) to express heterogeneous fusion protein ( MBP-mHD-5 ) .
	manualset3
159127	2	411557	7	NULL	NULL	0	NULL	engineered strain BL21 ( DE3 )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasmid pMAL-p2x-mHD-5 was transferred into engineered strain BL21 ( DE3 ) to express heterogeneous fusion protein ( MBP-mHD-5 ) .
	manualset3
159128	3	411557	7	NULL	NULL	0	NULL	heterogeneous fusion protein ( MBP-mHD-5 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasmid pMAL-p2x-mHD-5 was transferred into engineered strain BL21 ( DE3 ) to express heterogeneous fusion protein ( MBP-mHD-5 ) .
	manualset3
159129	1	411558	7	NULL	NULL	0	NULL	plasmid 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasmid was transformed into strains of S. gordonii expressing the fusion protein SpaP/S1 , the anti-complement receptor 1 ( CR1 ) single-chain variable fragment ( scFv ) antibody , or the Toxoplasma gondii cyclophilin C18 protein .
	manualset3
159130	2	411558	7	NULL	NULL	0	NULL	strains of S. gordonii	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasmid was transformed into strains of S. gordonii expressing the fusion protein SpaP/S1 , the anti-complement receptor 1 ( CR1 ) single-chain variable fragment ( scFv ) antibody , or the Toxoplasma gondii cyclophilin C18 protein .
	manualset3
159131	3	411558	7	NULL	NULL	0	NULL	fusion protein SpaP/S1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasmid was transformed into strains of S. gordonii expressing the fusion protein SpaP/S1 , the anti-complement receptor 1 ( CR1 ) single-chain variable fragment ( scFv ) antibody , or the Toxoplasma gondii cyclophilin C18 protein .
	manualset3
159132	4	411558	7	NULL	NULL	NULL	NULL	anti-complement receptor 1 ( CR1 ) single-chain variable fragment ( scFv ) antibody	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The plasmid was transformed into strains of S. gordonii expressing the fusion protein SpaP/S1 , the anti-complement receptor 1 ( CR1 ) single-chain variable fragment ( scFv ) antibody , or the Toxoplasma gondii cyclophilin C18 protein .
	manualset3
159133	5	411558	7	NULL	NULL	0	NULL	Toxoplasma gondii cyclophilin C18 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The plasmid was transformed into strains of S. gordonii expressing the fusion protein SpaP/S1 , the anti-complement receptor 1 ( CR1 ) single-chain variable fragment ( scFv ) antibody , or the Toxoplasma gondii cyclophilin C18 protein .
	manualset3
159134	1	411559	7	NULL	NULL	NULL	NULL	plastic tail grip 	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The plastic tail grip of the PLL will not release the tail end of the suture material before either the suture material or the slip knot fails .
	manualset3
159135	3	411559	7	NULL	NULL	NULL	NULL	tail end 	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The plastic tail grip of the PLL will not release the tail end of the suture material before either the suture material or the slip knot fails .
	manualset3
159137	6	411559	7	NULL	NULL	NULL	NULL	slip knot	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The plastic tail grip of the PLL will not release the tail end of the suture material before either the suture material or the slip knot fails .
	manualset3
160310	2	411559	7	NULL	NULL	NULL	NULL	 PLL 	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The plastic tail grip of the PLL will not release the tail end of the suture material before either the suture material or the slip knot fails .
	manualset3
160311	4	411559	7	NULL	NULL	NULL	NULL	suture material	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The plastic tail grip of the PLL will not release the tail end of the suture material before either the suture material or the slip knot fails .
	manualset3
160312	5	411559	7	NULL	NULL	0	NULL	suture material	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The plastic tail grip of the PLL will not release the tail end of the suture material before either the suture material or the slip knot fails .
	manualset3
159138	1	411560	7	NULL	NULL	0	NULL	pneumopathogenicity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The pneumopathogenicity of a trypsin-sensitive revertant of Sendai virus , TSrev-58 , which was derived from a trypsin-resistant mutant , TR-5 , was examined in mice .
	manualset3
159139	2	411560	7	NULL	NULL	0	NULL	trypsin-sensitive revertant of Sendai virus , TSrev-58 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The pneumopathogenicity of a trypsin-sensitive revertant of Sendai virus , TSrev-58 , which was derived from a trypsin-resistant mutant , TR-5 , was examined in mice .
	manualset3
159140	3	411560	7	NULL	NULL	0	NULL	trypsin-resistant mutant , TR-5	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The pneumopathogenicity of a trypsin-sensitive revertant of Sendai virus , TSrev-58 , which was derived from a trypsin-resistant mutant , TR-5 , was examined in mice .
	manualset3
159141	4	411560	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The pneumopathogenicity of a trypsin-sensitive revertant of Sendai virus , TSrev-58 , which was derived from a trypsin-resistant mutant , TR-5 , was examined in mice .
	manualset3
159142	1	411561	7	NULL	NULL	0	NULL	polar accumulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The polar accumulation was comparable to that of methyl-accepting chemotaxis proteins ( MCPs ) and MCP-related proteins .
	manualset3
159143	2	411561	7	NULL	NULL	0	NULL	methyl-accepting chemotaxis proteins ( MCPs )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The polar accumulation was comparable to that of methyl-accepting chemotaxis proteins ( MCPs ) and MCP-related proteins .
	manualset3
159144	3	411561	7	NULL	NULL	NULL	NULL	MCP-related proteins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The polar accumulation was comparable to that of methyl-accepting chemotaxis proteins ( MCPs ) and MCP-related proteins .
	manualset3
159145	1	411562	7	NULL	NULL	0	NULL	policy implications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The policy implications described are of particular relevance for policymakers and industry practitioners in other Southeast Asian countries with similar health systems where governments have expressed interest in facilitating the growth of the medical tourist industry .
	manualset3
159146	2	411562	7	NULL	NULL	0	NULL	policymakers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The policy implications described are of particular relevance for policymakers and industry practitioners in other Southeast Asian countries with similar health systems where governments have expressed interest in facilitating the growth of the medical tourist industry .
	manualset3
159147	3	411562	7	NULL	NULL	0	NULL	industry practitioners	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The policy implications described are of particular relevance for policymakers and industry practitioners in other Southeast Asian countries with similar health systems where governments have expressed interest in facilitating the growth of the medical tourist industry .
	manualset3
159148	4	411562	7	NULL	NULL	0	NULL	Southeast Asian countries	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The policy implications described are of particular relevance for policymakers and industry practitioners in other Southeast Asian countries with similar health systems where governments have expressed interest in facilitating the growth of the medical tourist industry .
	manualset3
159149	5	411562	7	NULL	NULL	0	NULL	health systems	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The policy implications described are of particular relevance for policymakers and industry practitioners in other Southeast Asian countries with similar health systems where governments have expressed interest in facilitating the growth of the medical tourist industry .
	manualset3
159150	6	411562	7	NULL	NULL	0	NULL	governments 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The policy implications described are of particular relevance for policymakers and industry practitioners in other Southeast Asian countries with similar health systems where governments have expressed interest in facilitating the growth of the medical tourist industry .
	manualset3
159151	7	411562	7	NULL	NULL	0	NULL	interest	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The policy implications described are of particular relevance for policymakers and industry practitioners in other Southeast Asian countries with similar health systems where governments have expressed interest in facilitating the growth of the medical tourist industry .
	manualset3
159152	8	411562	7	NULL	NULL	0	NULL	growth	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The policy implications described are of particular relevance for policymakers and industry practitioners in other Southeast Asian countries with similar health systems where governments have expressed interest in facilitating the growth of the medical tourist industry .
	manualset3
159153	9	411562	7	NULL	NULL	0	NULL	medical tourist industry	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The policy implications described are of particular relevance for policymakers and industry practitioners in other Southeast Asian countries with similar health systems where governments have expressed interest in facilitating the growth of the medical tourist industry .
	manualset3
159154	1	411563	7	NULL	NULL	0	NULL	ALK expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	ALK expression was not associated with an improved progression-free or overall-survival in patients with systemic T-cell ALCL .
	manualset3
159155	2	411563	7	NULL	NULL	0	NULL	progression-free survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	ALK expression was not associated with an improved progression-free or overall-survival in patients with systemic T-cell ALCL .
	manualset3
159156	3	411563	7	NULL	NULL	0	NULL	overall-survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	ALK expression was not associated with an improved progression-free or overall-survival in patients with systemic T-cell ALCL .
	manualset3
159157	4	411563	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	ALK expression was not associated with an improved progression-free or overall-survival in patients with systemic T-cell ALCL .
	manualset3
159158	5	411563	7	NULL	NULL	0	NULL	systemic T-cell ALCL	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	ALK expression was not associated with an improved progression-free or overall-survival in patients with systemic T-cell ALCL .
	manualset3
159159	1	411564	7	NULL	NULL	0	NULL	polo-like protein kinases Fnk	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The polo-like protein kinases Fnk and Snk associate with a Ca ( 2 + ) - and integrin-binding protein and are regulated dynamically with synaptic plasticity .
	manualset3
159160	2	411564	7	NULL	NULL	0	NULL	 polo-like protein kinases Snk	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The polo-like protein kinases Fnk and Snk associate with a Ca ( 2 + ) - and integrin-binding protein and are regulated dynamically with synaptic plasticity .
	manualset3
159161	3	411564	7	NULL	NULL	0	NULL	Ca ( 2 + ) 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The polo-like protein kinases Fnk and Snk associate with a Ca ( 2 + ) - and integrin-binding protein and are regulated dynamically with synaptic plasticity .
	manualset3
159162	4	411564	7	NULL	NULL	0	NULL	integrin-binding protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The polo-like protein kinases Fnk and Snk associate with a Ca ( 2 + ) - and integrin-binding protein and are regulated dynamically with synaptic plasticity .
	manualset3
159163	5	411564	7	NULL	NULL	0	NULL	synaptic plasticity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The polo-like protein kinases Fnk and Snk associate with a Ca ( 2 + ) - and integrin-binding protein and are regulated dynamically with synaptic plasticity .
	manualset3
159164	1	411565	7	NULL	NULL	NULL	NULL	polyclonal IGF-I antiserum K 37	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The polyclonal IGF-I antiserum K 37 was characterized and demonstrated to be specific .
	manualset3
159165	1	411566	7	NULL	NULL	0	NULL	polycyclic aromatic hydrocarbon concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The polycyclic aromatic hydrocarbon concentrations in the eggs , collected from five nests after they were deserted , ranged from 21.20 ng/g to 461.08 ng/g , values which are high enough to cause the death of the embryos and poisoning of adult birds .
	manualset3
159166	2	411566	7	NULL	NULL	NULL	NULL	eggs	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The polycyclic aromatic hydrocarbon concentrations in the eggs , collected from five nests after they were deserted , ranged from 21.20 ng/g to 461.08 ng/g , values which are high enough to cause the death of the embryos and poisoning of adult birds .
	manualset3
159167	3	411566	7	NULL	NULL	0	NULL	five nests	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The polycyclic aromatic hydrocarbon concentrations in the eggs , collected from five nests after they were deserted , ranged from 21.20 ng/g to 461.08 ng/g , values which are high enough to cause the death of the embryos and poisoning of adult birds .
	manualset3
159168	4	411566	7	NULL	NULL	0	NULL	21.20 ng/g 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The polycyclic aromatic hydrocarbon concentrations in the eggs , collected from five nests after they were deserted , ranged from 21.20 ng/g to 461.08 ng/g , values which are high enough to cause the death of the embryos and poisoning of adult birds .
	manualset3
159169	5	411566	7	NULL	NULL	0	NULL	461.08 ng/g 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The polycyclic aromatic hydrocarbon concentrations in the eggs , collected from five nests after they were deserted , ranged from 21.20 ng/g to 461.08 ng/g , values which are high enough to cause the death of the embryos and poisoning of adult birds .
	manualset3
159170	6	411566	7	NULL	NULL	0	NULL	values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The polycyclic aromatic hydrocarbon concentrations in the eggs , collected from five nests after they were deserted , ranged from 21.20 ng/g to 461.08 ng/g , values which are high enough to cause the death of the embryos and poisoning of adult birds .
	manualset3
159172	7	411566	7	NULL	NULL	NULL	NULL	death of the embryos	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The polycyclic aromatic hydrocarbon concentrations in the eggs , collected from five nests after they were deserted , ranged from 21.20 ng/g to 461.08 ng/g , values which are high enough to cause the death of the embryos and poisoning of adult birds .
	manualset3
159173	8	411566	7	NULL	NULL	NULL	NULL	adult birds	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The polycyclic aromatic hydrocarbon concentrations in the eggs , collected from five nests after they were deserted , ranged from 21.20 ng/g to 461.08 ng/g , values which are high enough to cause the death of the embryos and poisoning of adult birds .
	manualset3
159174	1	411567	7	NULL	NULL	0	NULL	polyketal nanoparticles	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The polyketal nanoparticles are formulated from poly ( 1 , 4-phenyleneacetone dimethylene ketal ) ( PPADK ) , a new hydrophobic polymer which contains ketal linkages in its backbone .
	manualset3
159175	2	411567	7	NULL	NULL	0	NULL	 poly ( 1 , 4-phenyleneacetone dimethylene ketal ) ( PPADK )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The polyketal nanoparticles are formulated from poly ( 1 , 4-phenyleneacetone dimethylene ketal ) ( PPADK ) , a new hydrophobic polymer which contains ketal linkages in its backbone .
	manualset3
159176	3	411567	7	NULL	NULL	0	NULL	 hydrophobic polymer 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The polyketal nanoparticles are formulated from poly ( 1 , 4-phenyleneacetone dimethylene ketal ) ( PPADK ) , a new hydrophobic polymer which contains ketal linkages in its backbone .
	manualset3
159177	4	411567	7	NULL	NULL	NULL	NULL	ketal linkages 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The polyketal nanoparticles are formulated from poly ( 1 , 4-phenyleneacetone dimethylene ketal ) ( PPADK ) , a new hydrophobic polymer which contains ketal linkages in its backbone .
	manualset3
159178	5	411567	7	NULL	NULL	0	NULL	backbone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The polyketal nanoparticles are formulated from poly ( 1 , 4-phenyleneacetone dimethylene ketal ) ( PPADK ) , a new hydrophobic polymer which contains ketal linkages in its backbone .
	manualset3
159179	1	411568	7	NULL	NULL	0	NULL	polymer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The polymer used was poly ( epsilon-caprolactone ) and the model protein was bovine serum albumin .
	manualset3
159180	2	411568	7	NULL	NULL	0	NULL	poly ( epsilon-caprolactone )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The polymer used was poly ( epsilon-caprolactone ) and the model protein was bovine serum albumin .
	manualset3
159181	3	411568	7	NULL	NULL	0	NULL	model protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The polymer used was poly ( epsilon-caprolactone ) and the model protein was bovine serum albumin .
	manualset3
159182	4	411568	7	NULL	NULL	0	NULL	bovine serum albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The polymer used was poly ( epsilon-caprolactone ) and the model protein was bovine serum albumin .
	manualset3
159183	1	411569	7	NULL	NULL	0	NULL	polymerase chain reaction 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The polymerase chain reaction was used to generate a rat E-selectin cDNA fragment by using heart total RNA from rats exposed to LPS .
	manualset3
159184	2	411569	7	NULL	NULL	0	NULL	 rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The polymerase chain reaction was used to generate a rat E-selectin cDNA fragment by using heart total RNA from rats exposed to LPS .
	manualset3
159185	3	411569	7	NULL	NULL	0	NULL	E-selectin cDNA fragment	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The polymerase chain reaction was used to generate a rat E-selectin cDNA fragment by using heart total RNA from rats exposed to LPS .
	manualset3
159186	4	411569	7	NULL	NULL	0	NULL	heart total RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The polymerase chain reaction was used to generate a rat E-selectin cDNA fragment by using heart total RNA from rats exposed to LPS .
	manualset3
159187	5	411569	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The polymerase chain reaction was used to generate a rat E-selectin cDNA fragment by using heart total RNA from rats exposed to LPS .
	manualset3
159188	6	411569	7	NULL	NULL	0	NULL	LPS	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The polymerase chain reaction was used to generate a rat E-selectin cDNA fragment by using heart total RNA from rats exposed to LPS .
	manualset3
159189	1	411570	7	NULL	NULL	NULL	NULL	 polymorphic nature 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The polymorphic nature of protein aggregation could be magnified in the cross-seeding process .
	manualset3
159190	3	411570	7	NULL	NULL	NULL	NULL	cross-seeding process	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The polymorphic nature of protein aggregation could be magnified in the cross-seeding process .
	manualset3
160313	2	411570	7	NULL	NULL	0	NULL	protein aggregation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The polymorphic nature of protein aggregation could be magnified in the cross-seeding process .
	manualset3
159191	1	411571	7	NULL	NULL	0	NULL	 polymorphism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The polymorphism -308 and -238 were revealed by restriction fragment length polymorphism ( RFLP ; NCOI and MSPI ) after the promoter site was amplified by PCR .
	manualset3
159192	2	411571	7	NULL	NULL	0	NULL	-308	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The polymorphism -308 and -238 were revealed by restriction fragment length polymorphism ( RFLP ; NCOI and MSPI ) after the promoter site was amplified by PCR .
	manualset3
159193	3	411571	7	NULL	NULL	0	NULL	-238 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The polymorphism -308 and -238 were revealed by restriction fragment length polymorphism ( RFLP ; NCOI and MSPI ) after the promoter site was amplified by PCR .
	manualset3
159194	4	411571	7	NULL	NULL	0	NULL	restriction fragment length polymorphism ( RFLP ; NCOI and MSPI )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The polymorphism -308 and -238 were revealed by restriction fragment length polymorphism ( RFLP ; NCOI and MSPI ) after the promoter site was amplified by PCR .
	manualset3
159195	5	411571	7	NULL	NULL	0	NULL	promoter site 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The polymorphism -308 and -238 were revealed by restriction fragment length polymorphism ( RFLP ; NCOI and MSPI ) after the promoter site was amplified by PCR .
	manualset3
159196	6	411571	7	NULL	NULL	0	NULL	PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The polymorphism -308 and -238 were revealed by restriction fragment length polymorphism ( RFLP ; NCOI and MSPI ) after the promoter site was amplified by PCR .
	manualset3
159197	1	411572	7	NULL	NULL	0	NULL	polypeptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The polypeptides and pig brain tubulin subunits were partially digested with S. aureus V8 protease , and the peptides obtained analysis by SDS-polyacrylamide gel electrophoresis .
	manualset3
159198	2	411572	7	NULL	NULL	0	NULL	 pig brain tubulin subunits	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The polypeptides and pig brain tubulin subunits were partially digested with S. aureus V8 protease , and the peptides obtained analysis by SDS-polyacrylamide gel electrophoresis .
	manualset3
159199	3	411572	7	NULL	NULL	0	NULL	S. aureus V8 protease	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The polypeptides and pig brain tubulin subunits were partially digested with S. aureus V8 protease , and the peptides obtained analysis by SDS-polyacrylamide gel electrophoresis .
	manualset3
159200	4	411572	7	NULL	NULL	0	NULL	peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The polypeptides and pig brain tubulin subunits were partially digested with S. aureus V8 protease , and the peptides obtained analysis by SDS-polyacrylamide gel electrophoresis .
	manualset3
159201	5	411572	7	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The polypeptides and pig brain tubulin subunits were partially digested with S. aureus V8 protease , and the peptides obtained analysis by SDS-polyacrylamide gel electrophoresis .
	manualset3
159202	6	411572	7	NULL	NULL	0	NULL	SDS-polyacrylamide gel electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The polypeptides and pig brain tubulin subunits were partially digested with S. aureus V8 protease , and the peptides obtained analysis by SDS-polyacrylamide gel electrophoresis .
	manualset3
159203	1	411573	7	NULL	NULL	0	NULL	polysorbates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The polysorbates undergo autooxidation , cleavage at the ethylene oxide subunits and hydrolysis of the fatty acid ester bond .
	manualset3
159204	2	411573	7	NULL	NULL	NULL	NULL	autooxidation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The polysorbates undergo autooxidation , cleavage at the ethylene oxide subunits and hydrolysis of the fatty acid ester bond .
	manualset3
159205	3	411573	7	NULL	NULL	NULL	NULL	cleavage	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The polysorbates undergo autooxidation , cleavage at the ethylene oxide subunits and hydrolysis of the fatty acid ester bond .
	manualset3
159206	4	411573	7	NULL	NULL	0	NULL	ethylene oxide subunits	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The polysorbates undergo autooxidation , cleavage at the ethylene oxide subunits and hydrolysis of the fatty acid ester bond .
	manualset3
159207	5	411573	7	NULL	NULL	NULL	NULL	hydrolysis	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The polysorbates undergo autooxidation , cleavage at the ethylene oxide subunits and hydrolysis of the fatty acid ester bond .
	manualset3
159208	6	411573	7	NULL	NULL	0	NULL	 fatty acid ester bond 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The polysorbates undergo autooxidation , cleavage at the ethylene oxide subunits and hydrolysis of the fatty acid ester bond .
	manualset3
159209	1	411574	7	NULL	NULL	NULL	NULL	ALP	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ALP showed progressively higher expression with increasing US intensities , whereas OP responded differently , showing down-regulation at 120 mW/cm2 , the lowest US exposure .
	manualset3
159210	2	411574	7	NULL	NULL	NULL	NULL	increasing US intensities	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ALP showed progressively higher expression with increasing US intensities , whereas OP responded differently , showing down-regulation at 120 mW/cm2 , the lowest US exposure .
	manualset3
159211	3	411574	7	NULL	NULL	0	NULL	OP	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	ALP showed progressively higher expression with increasing US intensities , whereas OP responded differently , showing down-regulation at 120 mW/cm2 , the lowest US exposure .
	manualset3
159212	4	411574	7	NULL	NULL	0	NULL	down-regulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	ALP showed progressively higher expression with increasing US intensities , whereas OP responded differently , showing down-regulation at 120 mW/cm2 , the lowest US exposure .
	manualset3
159213	5	411574	7	NULL	NULL	0	NULL	120 mW/cm2 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	ALP showed progressively higher expression with increasing US intensities , whereas OP responded differently , showing down-regulation at 120 mW/cm2 , the lowest US exposure .
	manualset3
159214	6	411574	7	NULL	NULL	0	NULL	 lowest US exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	ALP showed progressively higher expression with increasing US intensities , whereas OP responded differently , showing down-regulation at 120 mW/cm2 , the lowest US exposure .
	manualset3
162697	7	411574	7	NULL	NULL	NULL	NULL	expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ALP showed progressively higher expression with increasing US intensities , whereas OP responded differently , showing down-regulation at 120 mW/cm2 , the lowest US exposure .
	manualset3
159215	1	411575	7	NULL	NULL	0	NULL	pool size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The pool size of esterified and non-esterified fatty acids of WAT was reduced in both the well-fed animals raised in the cold and in the starving ones .
	manualset3
159216	2	411575	7	NULL	NULL	0	NULL	esterified and non-esterified fatty acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The pool size of esterified and non-esterified fatty acids of WAT was reduced in both the well-fed animals raised in the cold and in the starving ones .
	manualset3
159217	3	411575	7	NULL	NULL	0	NULL	WAT	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The pool size of esterified and non-esterified fatty acids of WAT was reduced in both the well-fed animals raised in the cold and in the starving ones .
	manualset3
159218	4	411575	7	NULL	NULL	0	NULL	well-fed animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The pool size of esterified and non-esterified fatty acids of WAT was reduced in both the well-fed animals raised in the cold and in the starving ones .
	manualset3
159219	5	411575	7	NULL	NULL	NULL	NULL	cold	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The pool size of esterified and non-esterified fatty acids of WAT was reduced in both the well-fed animals raised in the cold and in the starving ones .
	manualset3
159220	6	411575	7	NULL	NULL	NULL	NULL	starving ones	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The pool size of esterified and non-esterified fatty acids of WAT was reduced in both the well-fed animals raised in the cold and in the starving ones .
	manualset3
159221	1	411576	7	NULL	NULL	0	NULL	pooled ORs	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The pooled ORs for GSTT1 null genotype were 1.03 ( 95 % CI = 0.71-1 .49 ) in population-based studies and 2.39 ( 95 % CI = 0.73-7 .86 ) in hospital-based studies , stratifying for study design .
	manualset3
159222	2	411576	7	NULL	NULL	0	NULL	GSTT1 null genotype	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The pooled ORs for GSTT1 null genotype were 1.03 ( 95 % CI = 0.71-1 .49 ) in population-based studies and 2.39 ( 95 % CI = 0.73-7 .86 ) in hospital-based studies , stratifying for study design .
	manualset3
159223	3	411576	7	NULL	NULL	0	NULL	1.03 ( 95 % CI = 0.71-1 .49 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The pooled ORs for GSTT1 null genotype were 1.03 ( 95 % CI = 0.71-1 .49 ) in population-based studies and 2.39 ( 95 % CI = 0.73-7 .86 ) in hospital-based studies , stratifying for study design .
	manualset3
159224	4	411576	7	NULL	NULL	0	NULL	population-based studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The pooled ORs for GSTT1 null genotype were 1.03 ( 95 % CI = 0.71-1 .49 ) in population-based studies and 2.39 ( 95 % CI = 0.73-7 .86 ) in hospital-based studies , stratifying for study design .
	manualset3
159225	5	411576	7	NULL	NULL	0	NULL	2.39 ( 95 % CI = 0.73-7 .86 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The pooled ORs for GSTT1 null genotype were 1.03 ( 95 % CI = 0.71-1 .49 ) in population-based studies and 2.39 ( 95 % CI = 0.73-7 .86 ) in hospital-based studies , stratifying for study design .
	manualset3
159226	6	411576	7	NULL	NULL	0	NULL	hospital-based studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The pooled ORs for GSTT1 null genotype were 1.03 ( 95 % CI = 0.71-1 .49 ) in population-based studies and 2.39 ( 95 % CI = 0.73-7 .86 ) in hospital-based studies , stratifying for study design .
	manualset3
159227	7	411576	7	NULL	NULL	0	NULL	study design	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The pooled ORs for GSTT1 null genotype were 1.03 ( 95 % CI = 0.71-1 .49 ) in population-based studies and 2.39 ( 95 % CI = 0.73-7 .86 ) in hospital-based studies , stratifying for study design .
	manualset3
159228	1	411577	7	NULL	NULL	0	NULL	popularity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The popularity of the co-dependency concept has grown rapidly in the alcoholism treatment field .
	manualset3
159229	2	411577	7	NULL	NULL	0	NULL	 co-dependency concept	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The popularity of the co-dependency concept has grown rapidly in the alcoholism treatment field .
	manualset3
159230	3	411577	7	NULL	NULL	NULL	NULL	alcoholism treatment field 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The popularity of the co-dependency concept has grown rapidly in the alcoholism treatment field .
	manualset3
159231	1	411578	7	NULL	NULL	0	NULL	population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The population consisted of 55 self-identified light to heavy drinkers .
	manualset3
159232	2	411578	7	NULL	NULL	0	NULL	55	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The population consisted of 55 self-identified light to heavy drinkers .
	manualset3
159233	3	411578	7	NULL	NULL	NULL	NULL	light to heavy drinkers	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The population consisted of 55 self-identified light to heavy drinkers .
	manualset3
159234	1	411579	7	NULL	NULL	NULL	NULL	position 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The position of dorsal horn seems itself to depend on unequal or differential growth of the basal part of the ventricular ampullae .
	manualset3
159235	2	411579	7	NULL	NULL	0	NULL	dorsal horn	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The position of dorsal horn seems itself to depend on unequal or differential growth of the basal part of the ventricular ampullae .
	manualset3
159236	3	411579	7	NULL	NULL	NULL	NULL	unequal  growth 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The position of dorsal horn seems itself to depend on unequal or differential growth of the basal part of the ventricular ampullae .
	manualset3
159237	5	411579	7	NULL	NULL	NULL	NULL	basal part of the ventricular ampullae	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The position of dorsal horn seems itself to depend on unequal or differential growth of the basal part of the ventricular ampullae .
	manualset3
160314	4	411579	7	NULL	NULL	0	NULL	differential growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The position of dorsal horn seems itself to depend on unequal or differential growth of the basal part of the ventricular ampullae .
	manualset3
159238	1	411580	7	NULL	NULL	NULL	NULL	 introns	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The position of introns and similarities in the nucleic acid and amino acid sequences of the different classes of ADH enzymes in plants and humans suggest that plant and animal class III enzymes diverged before they duplicated to give rise to plant and animal ethanol-active ADH enzymes .
	manualset3
159239	2	411580	7	NULL	NULL	NULL	NULL	similarities	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The position of introns and similarities in the nucleic acid and amino acid sequences of the different classes of ADH enzymes in plants and humans suggest that plant and animal class III enzymes diverged before they duplicated to give rise to plant and animal ethanol-active ADH enzymes .
	manualset3
159240	3	411580	7	NULL	NULL	0	NULL	nucleic acid	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The position of introns and similarities in the nucleic acid and amino acid sequences of the different classes of ADH enzymes in plants and humans suggest that plant and animal class III enzymes diverged before they duplicated to give rise to plant and animal ethanol-active ADH enzymes .
	manualset3
159241	4	411580	7	NULL	NULL	0	NULL	amino acid sequences 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The position of introns and similarities in the nucleic acid and amino acid sequences of the different classes of ADH enzymes in plants and humans suggest that plant and animal class III enzymes diverged before they duplicated to give rise to plant and animal ethanol-active ADH enzymes .
	manualset3
159242	5	411580	7	NULL	NULL	NULL	NULL	different classes of ADH enzymes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The position of introns and similarities in the nucleic acid and amino acid sequences of the different classes of ADH enzymes in plants and humans suggest that plant and animal class III enzymes diverged before they duplicated to give rise to plant and animal ethanol-active ADH enzymes .
	manualset3
159243	6	411580	7	NULL	NULL	0	NULL	 plants 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The position of introns and similarities in the nucleic acid and amino acid sequences of the different classes of ADH enzymes in plants and humans suggest that plant and animal class III enzymes diverged before they duplicated to give rise to plant and animal ethanol-active ADH enzymes .
	manualset3
159244	7	411580	7	NULL	NULL	0	NULL	humans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The position of introns and similarities in the nucleic acid and amino acid sequences of the different classes of ADH enzymes in plants and humans suggest that plant and animal class III enzymes diverged before they duplicated to give rise to plant and animal ethanol-active ADH enzymes .
	manualset3
159245	8	411580	7	NULL	NULL	NULL	NULL	 class III enzymes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The position of introns and similarities in the nucleic acid and amino acid sequences of the different classes of ADH enzymes in plants and humans suggest that plant and animal class III enzymes diverged before they duplicated to give rise to plant and animal ethanol-active ADH enzymes .
	manualset3
159246	9	411580	7	NULL	NULL	0	NULL	plant 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The position of introns and similarities in the nucleic acid and amino acid sequences of the different classes of ADH enzymes in plants and humans suggest that plant and animal class III enzymes diverged before they duplicated to give rise to plant and animal ethanol-active ADH enzymes .
	manualset3
159247	10	411580	7	NULL	NULL	0	NULL	animal	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The position of introns and similarities in the nucleic acid and amino acid sequences of the different classes of ADH enzymes in plants and humans suggest that plant and animal class III enzymes diverged before they duplicated to give rise to plant and animal ethanol-active ADH enzymes .
	manualset3
159248	11	411580	7	NULL	NULL	0	NULL	ethanol-active ADH enzymes	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The position of introns and similarities in the nucleic acid and amino acid sequences of the different classes of ADH enzymes in plants and humans suggest that plant and animal class III enzymes diverged before they duplicated to give rise to plant and animal ethanol-active ADH enzymes .
	manualset3
160315	12	411580	7	NULL	NULL	0	NULL	position	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The position of introns and similarities in the nucleic acid and amino acid sequences of the different classes of ADH enzymes in plants and humans suggest that plant and animal class III enzymes diverged before they duplicated to give rise to plant and animal ethanol-active ADH enzymes .
	manualset3
159249	1	411581	7	NULL	NULL	0	NULL	 position	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The position of the chief of nursing practice is a role model for nursing leadership and one that is pivotal for the professional identity of nursing , and for the provision of high quality patient care .
	manualset3
159250	2	411581	7	NULL	NULL	NULL	NULL	chief 	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The position of the chief of nursing practice is a role model for nursing leadership and one that is pivotal for the professional identity of nursing , and for the provision of high quality patient care .
	manualset3
159251	3	411581	7	NULL	NULL	0	NULL	role model	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The position of the chief of nursing practice is a role model for nursing leadership and one that is pivotal for the professional identity of nursing , and for the provision of high quality patient care .
	manualset3
159252	4	411581	7	NULL	NULL	NULL	NULL	nursing leadership	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The position of the chief of nursing practice is a role model for nursing leadership and one that is pivotal for the professional identity of nursing , and for the provision of high quality patient care .
	manualset3
159253	5	411581	7	NULL	NULL	NULL	NULL	professional identity 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The position of the chief of nursing practice is a role model for nursing leadership and one that is pivotal for the professional identity of nursing , and for the provision of high quality patient care .
	manualset3
159255	7	411581	7	NULL	NULL	0	NULL	high quality patient care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The position of the chief of nursing practice is a role model for nursing leadership and one that is pivotal for the professional identity of nursing , and for the provision of high quality patient care .
	manualset3
160316	8	411581	7	NULL	NULL	NULL	NULL	nursing practice	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The position of the chief of nursing practice is a role model for nursing leadership and one that is pivotal for the professional identity of nursing , and for the provision of high quality patient care .
	manualset3
159256	1	411582	7	NULL	NULL	NULL	NULL	 position	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The position of the cross-linked lysine was only three amino acid residues away from the invariant proline residue mapped as the S-1-rod hinge by McLachlan and Karn ( McLachlan , A. D. , & Karn , J. ( 1982 ) Nature ( London ) 299 , 226-231 ) .
	manualset3
159257	2	411582	7	NULL	NULL	0	NULL	cross-linked lysine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The position of the cross-linked lysine was only three amino acid residues away from the invariant proline residue mapped as the S-1-rod hinge by McLachlan and Karn ( McLachlan , A. D. , & Karn , J. ( 1982 ) Nature ( London ) 299 , 226-231 ) .
	manualset3
159258	3	411582	7	NULL	NULL	0	NULL	three amino acid residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The position of the cross-linked lysine was only three amino acid residues away from the invariant proline residue mapped as the S-1-rod hinge by McLachlan and Karn ( McLachlan , A. D. , & Karn , J. ( 1982 ) Nature ( London ) 299 , 226-231 ) .
	manualset3
159259	4	411582	7	NULL	NULL	0	NULL	 invariant proline residue	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The position of the cross-linked lysine was only three amino acid residues away from the invariant proline residue mapped as the S-1-rod hinge by McLachlan and Karn ( McLachlan , A. D. , & Karn , J. ( 1982 ) Nature ( London ) 299 , 226-231 ) .
	manualset3
159260	5	411582	7	NULL	NULL	0	NULL	S-1-rod hinge	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The position of the cross-linked lysine was only three amino acid residues away from the invariant proline residue mapped as the S-1-rod hinge by McLachlan and Karn ( McLachlan , A. D. , & Karn , J. ( 1982 ) Nature ( London ) 299 , 226-231 ) .
	manualset3
159261	6	411582	7	NULL	NULL	0	NULL	McLachlan	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The position of the cross-linked lysine was only three amino acid residues away from the invariant proline residue mapped as the S-1-rod hinge by McLachlan and Karn ( McLachlan , A. D. , & Karn , J. ( 1982 ) Nature ( London ) 299 , 226-231 ) .
	manualset3
159262	7	411582	7	NULL	NULL	0	NULL	Karn	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The position of the cross-linked lysine was only three amino acid residues away from the invariant proline residue mapped as the S-1-rod hinge by McLachlan and Karn ( McLachlan , A. D. , & Karn , J. ( 1982 ) Nature ( London ) 299 , 226-231 ) .
	manualset3
159263	8	411582	7	NULL	NULL	0	NULL	McLachlan , A. D. , & Karn , J. ( 1982 ) Nature ( London ) 299 , 226-231 ) 	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	The position of the cross-linked lysine was only three amino acid residues away from the invariant proline residue mapped as the S-1-rod hinge by McLachlan and Karn ( McLachlan , A. D. , & Karn , J. ( 1982 ) Nature ( London ) 299 , 226-231 ) .
	manualset3
159264	1	411583	7	NULL	NULL	0	NULL	 position	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The position of two putative free-living trichomonads in the tree is indicative of derivation from symbionts rather than direct descent from some free-living ancestral trichomonad .
	manualset3
159265	2	411583	7	NULL	NULL	0	NULL	two putative free-living trichomonads 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The position of two putative free-living trichomonads in the tree is indicative of derivation from symbionts rather than direct descent from some free-living ancestral trichomonad .
	manualset3
159266	3	411583	7	NULL	NULL	0	NULL	tree	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The position of two putative free-living trichomonads in the tree is indicative of derivation from symbionts rather than direct descent from some free-living ancestral trichomonad .
	manualset3
159267	4	411583	7	NULL	NULL	0	NULL	derivation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The position of two putative free-living trichomonads in the tree is indicative of derivation from symbionts rather than direct descent from some free-living ancestral trichomonad .
	manualset3
159268	5	411583	7	NULL	NULL	0	NULL	symbionts	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The position of two putative free-living trichomonads in the tree is indicative of derivation from symbionts rather than direct descent from some free-living ancestral trichomonad .
	manualset3
159269	6	411583	7	NULL	NULL	0	NULL	 free-living ancestral trichomonad 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The position of two putative free-living trichomonads in the tree is indicative of derivation from symbionts rather than direct descent from some free-living ancestral trichomonad .
	manualset3
159270	1	411584	7	NULL	NULL	0	NULL	AM signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	AM signaling is of particular significance in endothelial cell biology since the peptide protects cells from apoptosis , promotes angiogenesis , and affects vascular tone and permeability .
	manualset3
159271	2	411584	7	NULL	NULL	0	NULL	endothelial cell biology 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	AM signaling is of particular significance in endothelial cell biology since the peptide protects cells from apoptosis , promotes angiogenesis , and affects vascular tone and permeability .
	manualset3
159272	3	411584	7	NULL	NULL	0	NULL	 peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	AM signaling is of particular significance in endothelial cell biology since the peptide protects cells from apoptosis , promotes angiogenesis , and affects vascular tone and permeability .
	manualset3
159273	4	411584	7	NULL	NULL	NULL	NULL	apoptosis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	AM signaling is of particular significance in endothelial cell biology since the peptide protects cells from apoptosis , promotes angiogenesis , and affects vascular tone and permeability .
	manualset3
159274	5	411584	7	NULL	NULL	NULL	NULL	angiogenesis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	AM signaling is of particular significance in endothelial cell biology since the peptide protects cells from apoptosis , promotes angiogenesis , and affects vascular tone and permeability .
	manualset3
159275	6	411584	7	NULL	NULL	NULL	NULL	vascular tone and permeability	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	AM signaling is of particular significance in endothelial cell biology since the peptide protects cells from apoptosis , promotes angiogenesis , and affects vascular tone and permeability .
	manualset3
159276	7	411584	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	AM signaling is of particular significance in endothelial cell biology since the peptide protects cells from apoptosis , promotes angiogenesis , and affects vascular tone and permeability .
	manualset3
159277	1	411585	7	NULL	NULL	0	NULL	position	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The position that dioxin causes human tumors remains a subject for debate ; however , recent epidemiological studies of a population highly exposed to dioxin in 1976 as a result of an industrial accident suggest that women with higher dioxin body burdens may have a lower incidence of breast cancer .
	manualset3
159278	2	411585	7	NULL	NULL	0	NULL	dioxin 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The position that dioxin causes human tumors remains a subject for debate ; however , recent epidemiological studies of a population highly exposed to dioxin in 1976 as a result of an industrial accident suggest that women with higher dioxin body burdens may have a lower incidence of breast cancer .
	manualset3
159279	3	411585	7	NULL	NULL	0	NULL	human tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The position that dioxin causes human tumors remains a subject for debate ; however , recent epidemiological studies of a population highly exposed to dioxin in 1976 as a result of an industrial accident suggest that women with higher dioxin body burdens may have a lower incidence of breast cancer .
	manualset3
159280	4	411585	7	NULL	NULL	0	NULL	subject	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The position that dioxin causes human tumors remains a subject for debate ; however , recent epidemiological studies of a population highly exposed to dioxin in 1976 as a result of an industrial accident suggest that women with higher dioxin body burdens may have a lower incidence of breast cancer .
	manualset3
159281	5	411585	7	NULL	NULL	0	NULL	debate	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The position that dioxin causes human tumors remains a subject for debate ; however , recent epidemiological studies of a population highly exposed to dioxin in 1976 as a result of an industrial accident suggest that women with higher dioxin body burdens may have a lower incidence of breast cancer .
	manualset3
159282	6	411585	7	NULL	NULL	0	NULL	epidemiological studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The position that dioxin causes human tumors remains a subject for debate ; however , recent epidemiological studies of a population highly exposed to dioxin in 1976 as a result of an industrial accident suggest that women with higher dioxin body burdens may have a lower incidence of breast cancer .
	manualset3
159283	7	411585	7	NULL	NULL	0	NULL	population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The position that dioxin causes human tumors remains a subject for debate ; however , recent epidemiological studies of a population highly exposed to dioxin in 1976 as a result of an industrial accident suggest that women with higher dioxin body burdens may have a lower incidence of breast cancer .
	manualset3
159284	8	411585	7	NULL	NULL	0	NULL	dioxin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The position that dioxin causes human tumors remains a subject for debate ; however , recent epidemiological studies of a population highly exposed to dioxin in 1976 as a result of an industrial accident suggest that women with higher dioxin body burdens may have a lower incidence of breast cancer .
	manualset3
159285	9	411585	7	NULL	NULL	NULL	NULL	1976	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The position that dioxin causes human tumors remains a subject for debate ; however , recent epidemiological studies of a population highly exposed to dioxin in 1976 as a result of an industrial accident suggest that women with higher dioxin body burdens may have a lower incidence of breast cancer .
	manualset3
159286	10	411585	7	NULL	NULL	0	NULL	industrial accident	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The position that dioxin causes human tumors remains a subject for debate ; however , recent epidemiological studies of a population highly exposed to dioxin in 1976 as a result of an industrial accident suggest that women with higher dioxin body burdens may have a lower incidence of breast cancer .
	manualset3
159287	11	411585	7	NULL	NULL	0	NULL	women	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The position that dioxin causes human tumors remains a subject for debate ; however , recent epidemiological studies of a population highly exposed to dioxin in 1976 as a result of an industrial accident suggest that women with higher dioxin body burdens may have a lower incidence of breast cancer .
	manualset3
159288	12	411585	7	NULL	NULL	NULL	NULL	dioxin body	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The position that dioxin causes human tumors remains a subject for debate ; however , recent epidemiological studies of a population highly exposed to dioxin in 1976 as a result of an industrial accident suggest that women with higher dioxin body burdens may have a lower incidence of breast cancer .
	manualset3
159289	13	411585	7	NULL	NULL	0	NULL	breast cancer	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The position that dioxin causes human tumors remains a subject for debate ; however , recent epidemiological studies of a population highly exposed to dioxin in 1976 as a result of an industrial accident suggest that women with higher dioxin body burdens may have a lower incidence of breast cancer .
	manualset3
162698	14	411585	7	NULL	NULL	0	NULL	result	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The position that dioxin causes human tumors remains a subject for debate ; however , recent epidemiological studies of a population highly exposed to dioxin in 1976 as a result of an industrial accident suggest that women with higher dioxin body burdens may have a lower incidence of breast cancer .
	manualset3
162699	15	411585	7	NULL	NULL	0	NULL	lower incidence 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The position that dioxin causes human tumors remains a subject for debate ; however , recent epidemiological studies of a population highly exposed to dioxin in 1976 as a result of an industrial accident suggest that women with higher dioxin body burdens may have a lower incidence of breast cancer .
	manualset3
159290	1	411586	7	NULL	NULL	0	NULL	 positive feedback effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The positive feedback effects of estradiol ( E2 ) and progesterone ( P ) on LH and FSH release were studied under novel experimental conditions in three women of reproductive age who had undergone oophorectomy and received uninterupted E2 replacement by subdermal implants .
	manualset3
159291	2	411586	7	NULL	NULL	0	NULL	estradiol ( E2 )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The positive feedback effects of estradiol ( E2 ) and progesterone ( P ) on LH and FSH release were studied under novel experimental conditions in three women of reproductive age who had undergone oophorectomy and received uninterupted E2 replacement by subdermal implants .
	manualset3
159292	3	411586	7	NULL	NULL	0	NULL	progesterone ( P )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The positive feedback effects of estradiol ( E2 ) and progesterone ( P ) on LH and FSH release were studied under novel experimental conditions in three women of reproductive age who had undergone oophorectomy and received uninterupted E2 replacement by subdermal implants .
	manualset3
159293	4	411586	7	NULL	NULL	NULL	NULL	LH release	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The positive feedback effects of estradiol ( E2 ) and progesterone ( P ) on LH and FSH release were studied under novel experimental conditions in three women of reproductive age who had undergone oophorectomy and received uninterupted E2 replacement by subdermal implants .
	manualset3
159294	5	411586	7	NULL	NULL	NULL	NULL	FSH release	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The positive feedback effects of estradiol ( E2 ) and progesterone ( P ) on LH and FSH release were studied under novel experimental conditions in three women of reproductive age who had undergone oophorectomy and received uninterupted E2 replacement by subdermal implants .
	manualset3
159295	6	411586	7	NULL	NULL	0	NULL	novel experimental conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The positive feedback effects of estradiol ( E2 ) and progesterone ( P ) on LH and FSH release were studied under novel experimental conditions in three women of reproductive age who had undergone oophorectomy and received uninterupted E2 replacement by subdermal implants .
	manualset3
159296	7	411586	7	NULL	NULL	0	NULL	three women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The positive feedback effects of estradiol ( E2 ) and progesterone ( P ) on LH and FSH release were studied under novel experimental conditions in three women of reproductive age who had undergone oophorectomy and received uninterupted E2 replacement by subdermal implants .
	manualset3
159297	8	411586	7	NULL	NULL	0	NULL	reproductive age	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The positive feedback effects of estradiol ( E2 ) and progesterone ( P ) on LH and FSH release were studied under novel experimental conditions in three women of reproductive age who had undergone oophorectomy and received uninterupted E2 replacement by subdermal implants .
	manualset3
159298	9	411586	7	NULL	NULL	0	NULL	oophorectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The positive feedback effects of estradiol ( E2 ) and progesterone ( P ) on LH and FSH release were studied under novel experimental conditions in three women of reproductive age who had undergone oophorectomy and received uninterupted E2 replacement by subdermal implants .
	manualset3
159299	10	411586	7	NULL	NULL	0	NULL	uninterupted E2 replacement	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The positive feedback effects of estradiol ( E2 ) and progesterone ( P ) on LH and FSH release were studied under novel experimental conditions in three women of reproductive age who had undergone oophorectomy and received uninterupted E2 replacement by subdermal implants .
	manualset3
159300	11	411586	7	NULL	NULL	0	NULL	subdermal implants	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The positive feedback effects of estradiol ( E2 ) and progesterone ( P ) on LH and FSH release were studied under novel experimental conditions in three women of reproductive age who had undergone oophorectomy and received uninterupted E2 replacement by subdermal implants .
	manualset3
159301	1	411587	7	NULL	NULL	0	NULL	positive predictive value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The positive predictive value for each test , used alone , for the identification of CMV pneumonitis was low .
	manualset3
159302	2	411587	7	NULL	NULL	0	NULL	test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The positive predictive value for each test , used alone , for the identification of CMV pneumonitis was low .
	manualset3
159303	3	411587	7	NULL	NULL	0	NULL	 identification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The positive predictive value for each test , used alone , for the identification of CMV pneumonitis was low .
	manualset3
159304	4	411587	7	NULL	NULL	0	NULL	CMV pneumonitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The positive predictive value for each test , used alone , for the identification of CMV pneumonitis was low .
	manualset3
159305	1	411588	7	NULL	NULL	0	NULL	positivities 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The positivities of serum ErbB-2 protein in patients with breast carcinoma were 13.0 % for primary cases and 47.9 % for recurrent cases .
	manualset3
159306	2	411588	7	NULL	NULL	0	NULL	serum ErbB-2 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The positivities of serum ErbB-2 protein in patients with breast carcinoma were 13.0 % for primary cases and 47.9 % for recurrent cases .
	manualset3
159307	3	411588	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The positivities of serum ErbB-2 protein in patients with breast carcinoma were 13.0 % for primary cases and 47.9 % for recurrent cases .
	manualset3
159308	4	411588	7	NULL	NULL	NULL	NULL	breast carcinoma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The positivities of serum ErbB-2 protein in patients with breast carcinoma were 13.0 % for primary cases and 47.9 % for recurrent cases .
	manualset3
159309	5	411588	7	NULL	NULL	0	NULL	13.0 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The positivities of serum ErbB-2 protein in patients with breast carcinoma were 13.0 % for primary cases and 47.9 % for recurrent cases .
	manualset3
159310	6	411588	7	NULL	NULL	0	NULL	primary cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The positivities of serum ErbB-2 protein in patients with breast carcinoma were 13.0 % for primary cases and 47.9 % for recurrent cases .
	manualset3
159311	7	411588	7	NULL	NULL	0	NULL	47.9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The positivities of serum ErbB-2 protein in patients with breast carcinoma were 13.0 % for primary cases and 47.9 % for recurrent cases .
	manualset3
159312	8	411588	7	NULL	NULL	0	NULL	recurrent cases 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The positivities of serum ErbB-2 protein in patients with breast carcinoma were 13.0 % for primary cases and 47.9 % for recurrent cases .
	manualset3
159313	1	411589	7	NULL	NULL	0	NULL	possibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility is shown of using LC to illustrate not only the surface but also the spacial configuration of a fingerprint .
	manualset3
159314	2	411589	7	NULL	NULL	0	NULL	LC	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility is shown of using LC to illustrate not only the surface but also the spacial configuration of a fingerprint .
	manualset3
159315	3	411589	7	NULL	NULL	0	NULL	surface	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility is shown of using LC to illustrate not only the surface but also the spacial configuration of a fingerprint .
	manualset3
159316	4	411589	7	NULL	NULL	0	NULL	spacial configuration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility is shown of using LC to illustrate not only the surface but also the spacial configuration of a fingerprint .
	manualset3
159317	5	411589	7	NULL	NULL	0	NULL	fingerprint	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility is shown of using LC to illustrate not only the surface but also the spacial configuration of a fingerprint .
	manualset3
159318	1	411590	7	NULL	NULL	0	NULL	possibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility of a description of acute and chronic pain therapy in the G-DRG system was initially rudimentary and not logically planned and also a fair allotment of proceeds according to resources was not possible .
	manualset3
159319	2	411590	7	NULL	NULL	0	NULL	description	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility of a description of acute and chronic pain therapy in the G-DRG system was initially rudimentary and not logically planned and also a fair allotment of proceeds according to resources was not possible .
	manualset3
159320	3	411590	7	NULL	NULL	0	NULL	acute  pain therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility of a description of acute and chronic pain therapy in the G-DRG system was initially rudimentary and not logically planned and also a fair allotment of proceeds according to resources was not possible .
	manualset3
159321	4	411590	7	NULL	NULL	0	NULL	chronic pain therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility of a description of acute and chronic pain therapy in the G-DRG system was initially rudimentary and not logically planned and also a fair allotment of proceeds according to resources was not possible .
	manualset3
159322	5	411590	7	NULL	NULL	NULL	NULL	G-DRG system 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The possibility of a description of acute and chronic pain therapy in the G-DRG system was initially rudimentary and not logically planned and also a fair allotment of proceeds according to resources was not possible .
	manualset3
159323	6	411590	7	NULL	NULL	0	NULL	fair allotment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility of a description of acute and chronic pain therapy in the G-DRG system was initially rudimentary and not logically planned and also a fair allotment of proceeds according to resources was not possible .
	manualset3
159324	7	411590	7	NULL	NULL	0	NULL	resources	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility of a description of acute and chronic pain therapy in the G-DRG system was initially rudimentary and not logically planned and also a fair allotment of proceeds according to resources was not possible .
	manualset3
159325	1	411591	7	NULL	NULL	0	NULL	 possibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility of nonspecific effects of ketanserin such as an interaction with alpha 1-adrenergic receptors merits careful evaluation , but in the case of the Class III effect , ketanserin was approximately 100 times more active than prazosin in widening the action potential duration .
	manualset3
159326	2	411591	7	NULL	NULL	0	NULL	nonspecific effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility of nonspecific effects of ketanserin such as an interaction with alpha 1-adrenergic receptors merits careful evaluation , but in the case of the Class III effect , ketanserin was approximately 100 times more active than prazosin in widening the action potential duration .
	manualset3
159327	3	411591	7	NULL	NULL	NULL	NULL	ketanserin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The possibility of nonspecific effects of ketanserin such as an interaction with alpha 1-adrenergic receptors merits careful evaluation , but in the case of the Class III effect , ketanserin was approximately 100 times more active than prazosin in widening the action potential duration .
	manualset3
159328	4	411591	7	NULL	NULL	0	NULL	interaction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility of nonspecific effects of ketanserin such as an interaction with alpha 1-adrenergic receptors merits careful evaluation , but in the case of the Class III effect , ketanserin was approximately 100 times more active than prazosin in widening the action potential duration .
	manualset3
159329	5	411591	7	NULL	NULL	0	NULL	alpha 1-adrenergic receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility of nonspecific effects of ketanserin such as an interaction with alpha 1-adrenergic receptors merits careful evaluation , but in the case of the Class III effect , ketanserin was approximately 100 times more active than prazosin in widening the action potential duration .
	manualset3
159330	6	411591	7	NULL	NULL	0	NULL	evaluation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility of nonspecific effects of ketanserin such as an interaction with alpha 1-adrenergic receptors merits careful evaluation , but in the case of the Class III effect , ketanserin was approximately 100 times more active than prazosin in widening the action potential duration .
	manualset3
159331	7	411591	7	NULL	NULL	0	NULL	Class III effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility of nonspecific effects of ketanserin such as an interaction with alpha 1-adrenergic receptors merits careful evaluation , but in the case of the Class III effect , ketanserin was approximately 100 times more active than prazosin in widening the action potential duration .
	manualset3
159332	8	411591	7	NULL	NULL	NULL	NULL	ketanserin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The possibility of nonspecific effects of ketanserin such as an interaction with alpha 1-adrenergic receptors merits careful evaluation , but in the case of the Class III effect , ketanserin was approximately 100 times more active than prazosin in widening the action potential duration .
	manualset3
159333	9	411591	7	NULL	NULL	NULL	NULL	100 times	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The possibility of nonspecific effects of ketanserin such as an interaction with alpha 1-adrenergic receptors merits careful evaluation , but in the case of the Class III effect , ketanserin was approximately 100 times more active than prazosin in widening the action potential duration .
	manualset3
159334	10	411591	7	NULL	NULL	NULL	NULL	prazosin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The possibility of nonspecific effects of ketanserin such as an interaction with alpha 1-adrenergic receptors merits careful evaluation , but in the case of the Class III effect , ketanserin was approximately 100 times more active than prazosin in widening the action potential duration .
	manualset3
159335	11	411591	7	NULL	NULL	NULL	NULL	action potential duration	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The possibility of nonspecific effects of ketanserin such as an interaction with alpha 1-adrenergic receptors merits careful evaluation , but in the case of the Class III effect , ketanserin was approximately 100 times more active than prazosin in widening the action potential duration .
	manualset3
159336	12	411591	7	NULL	NULL	NULL	NULL	widening	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The possibility of nonspecific effects of ketanserin such as an interaction with alpha 1-adrenergic receptors merits careful evaluation , but in the case of the Class III effect , ketanserin was approximately 100 times more active than prazosin in widening the action potential duration .
	manualset3
159337	1	411592	7	NULL	NULL	0	NULL	possibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility that neutrophils produce the hydroxyl radical ( OH - ) was studied by examining the ability of these cells to support the release of ethylene from methional , a reaction in which it has been shown that OH - , but not O2 - or H2O2 , may serve as the oxidizing agent .
	manualset3
159338	2	411592	7	NULL	NULL	0	NULL	neutrophils	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility that neutrophils produce the hydroxyl radical ( OH - ) was studied by examining the ability of these cells to support the release of ethylene from methional , a reaction in which it has been shown that OH - , but not O2 - or H2O2 , may serve as the oxidizing agent .
	manualset3
159339	3	411592	7	NULL	NULL	0	NULL	hydroxyl radical ( OH - )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility that neutrophils produce the hydroxyl radical ( OH - ) was studied by examining the ability of these cells to support the release of ethylene from methional , a reaction in which it has been shown that OH - , but not O2 - or H2O2 , may serve as the oxidizing agent .
	manualset3
159340	4	411592	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility that neutrophils produce the hydroxyl radical ( OH - ) was studied by examining the ability of these cells to support the release of ethylene from methional , a reaction in which it has been shown that OH - , but not O2 - or H2O2 , may serve as the oxidizing agent .
	manualset3
159341	5	411592	7	NULL	NULL	NULL	NULL	release of ethylene	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The possibility that neutrophils produce the hydroxyl radical ( OH - ) was studied by examining the ability of these cells to support the release of ethylene from methional , a reaction in which it has been shown that OH - , but not O2 - or H2O2 , may serve as the oxidizing agent .
	manualset3
159342	6	411592	7	NULL	NULL	0	NULL	methional	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility that neutrophils produce the hydroxyl radical ( OH - ) was studied by examining the ability of these cells to support the release of ethylene from methional , a reaction in which it has been shown that OH - , but not O2 - or H2O2 , may serve as the oxidizing agent .
	manualset3
159343	7	411592	7	NULL	NULL	0	NULL	reaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility that neutrophils produce the hydroxyl radical ( OH - ) was studied by examining the ability of these cells to support the release of ethylene from methional , a reaction in which it has been shown that OH - , but not O2 - or H2O2 , may serve as the oxidizing agent .
	manualset3
159344	8	411592	7	NULL	NULL	0	NULL	OH -	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility that neutrophils produce the hydroxyl radical ( OH - ) was studied by examining the ability of these cells to support the release of ethylene from methional , a reaction in which it has been shown that OH - , but not O2 - or H2O2 , may serve as the oxidizing agent .
	manualset3
159345	9	411592	7	NULL	NULL	0	NULL	O2 - 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility that neutrophils produce the hydroxyl radical ( OH - ) was studied by examining the ability of these cells to support the release of ethylene from methional , a reaction in which it has been shown that OH - , but not O2 - or H2O2 , may serve as the oxidizing agent .
	manualset3
159346	10	411592	7	NULL	NULL	0	NULL	H2O2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility that neutrophils produce the hydroxyl radical ( OH - ) was studied by examining the ability of these cells to support the release of ethylene from methional , a reaction in which it has been shown that OH - , but not O2 - or H2O2 , may serve as the oxidizing agent .
	manualset3
159347	11	411592	7	NULL	NULL	0	NULL	oxidizing agent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility that neutrophils produce the hydroxyl radical ( OH - ) was studied by examining the ability of these cells to support the release of ethylene from methional , a reaction in which it has been shown that OH - , but not O2 - or H2O2 , may serve as the oxidizing agent .
	manualset3
159348	1	411593	7	NULL	NULL	0	NULL	possibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility that some of these muscarinic receptors may be involved in regulation of phosphinositide metabolism and the protein kinase activities of myelin is considered .
	manualset3
159349	2	411593	7	NULL	NULL	0	NULL	muscarinic receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility that some of these muscarinic receptors may be involved in regulation of phosphinositide metabolism and the protein kinase activities of myelin is considered .
	manualset3
159350	3	411593	7	NULL	NULL	0	NULL	regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility that some of these muscarinic receptors may be involved in regulation of phosphinositide metabolism and the protein kinase activities of myelin is considered .
	manualset3
159351	4	411593	7	NULL	NULL	0	NULL	phosphinositide metabolism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility that some of these muscarinic receptors may be involved in regulation of phosphinositide metabolism and the protein kinase activities of myelin is considered .
	manualset3
159352	5	411593	7	NULL	NULL	0	NULL	protein kinase activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility that some of these muscarinic receptors may be involved in regulation of phosphinositide metabolism and the protein kinase activities of myelin is considered .
	manualset3
159353	6	411593	7	NULL	NULL	0	NULL	myelin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility that some of these muscarinic receptors may be involved in regulation of phosphinositide metabolism and the protein kinase activities of myelin is considered .
	manualset3
159354	1	411594	7	NULL	NULL	0	NULL	 possibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility that the involved PDE was calcium sensitive was assessed ; during PDE inhibition by Ro 20-1724 , but not by IBMX , calcium ionophore A23187 inhibited PTH-stimulated cAMP accumulation and PMA abolished the effect of A23187 .
	manualset3
159355	2	411594	7	NULL	NULL	0	NULL	PDE	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility that the involved PDE was calcium sensitive was assessed ; during PDE inhibition by Ro 20-1724 , but not by IBMX , calcium ionophore A23187 inhibited PTH-stimulated cAMP accumulation and PMA abolished the effect of A23187 .
	manualset3
159356	3	411594	7	NULL	NULL	NULL	NULL	calcium 	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The possibility that the involved PDE was calcium sensitive was assessed ; during PDE inhibition by Ro 20-1724 , but not by IBMX , calcium ionophore A23187 inhibited PTH-stimulated cAMP accumulation and PMA abolished the effect of A23187 .
	manualset3
159357	4	411594	7	NULL	NULL	NULL	NULL	PDE inhibition	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The possibility that the involved PDE was calcium sensitive was assessed ; during PDE inhibition by Ro 20-1724 , but not by IBMX , calcium ionophore A23187 inhibited PTH-stimulated cAMP accumulation and PMA abolished the effect of A23187 .
	manualset3
159358	5	411594	7	NULL	NULL	0	NULL	Ro 20-1724	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility that the involved PDE was calcium sensitive was assessed ; during PDE inhibition by Ro 20-1724 , but not by IBMX , calcium ionophore A23187 inhibited PTH-stimulated cAMP accumulation and PMA abolished the effect of A23187 .
	manualset3
159359	6	411594	7	NULL	NULL	0	NULL	IBMX	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility that the involved PDE was calcium sensitive was assessed ; during PDE inhibition by Ro 20-1724 , but not by IBMX , calcium ionophore A23187 inhibited PTH-stimulated cAMP accumulation and PMA abolished the effect of A23187 .
	manualset3
159360	7	411594	7	NULL	NULL	0	NULL	calcium ionophore A23187	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility that the involved PDE was calcium sensitive was assessed ; during PDE inhibition by Ro 20-1724 , but not by IBMX , calcium ionophore A23187 inhibited PTH-stimulated cAMP accumulation and PMA abolished the effect of A23187 .
	manualset3
159361	8	411594	7	NULL	NULL	0	NULL	PTH-stimulated cAMP accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility that the involved PDE was calcium sensitive was assessed ; during PDE inhibition by Ro 20-1724 , but not by IBMX , calcium ionophore A23187 inhibited PTH-stimulated cAMP accumulation and PMA abolished the effect of A23187 .
	manualset3
159362	9	411594	7	NULL	NULL	0	NULL	PMA	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility that the involved PDE was calcium sensitive was assessed ; during PDE inhibition by Ro 20-1724 , but not by IBMX , calcium ionophore A23187 inhibited PTH-stimulated cAMP accumulation and PMA abolished the effect of A23187 .
	manualset3
159363	10	411594	7	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility that the involved PDE was calcium sensitive was assessed ; during PDE inhibition by Ro 20-1724 , but not by IBMX , calcium ionophore A23187 inhibited PTH-stimulated cAMP accumulation and PMA abolished the effect of A23187 .
	manualset3
159364	11	411594	7	NULL	NULL	0	NULL	A23187	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The possibility that the involved PDE was calcium sensitive was assessed ; during PDE inhibition by Ro 20-1724 , but not by IBMX , calcium ionophore A23187 inhibited PTH-stimulated cAMP accumulation and PMA abolished the effect of A23187 .
	manualset3
159365	1	411595	7	NULL	NULL	NULL	NULL	possible dissociation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The possible dissociation of LHC I as an early structural change in the PS I complex after DDC-induced photoinhibition of PS I is discussed .
	manualset3
159366	2	411595	7	NULL	NULL	0	NULL	LHC I 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible dissociation of LHC I as an early structural change in the PS I complex after DDC-induced photoinhibition of PS I is discussed .
	manualset3
159367	3	411595	7	NULL	NULL	0	NULL	early structural change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible dissociation of LHC I as an early structural change in the PS I complex after DDC-induced photoinhibition of PS I is discussed .
	manualset3
159368	4	411595	7	NULL	NULL	0	NULL	PS I complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible dissociation of LHC I as an early structural change in the PS I complex after DDC-induced photoinhibition of PS I is discussed .
	manualset3
159369	5	411595	7	NULL	NULL	0	NULL	DDC-induced photoinhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible dissociation of LHC I as an early structural change in the PS I complex after DDC-induced photoinhibition of PS I is discussed .
	manualset3
159370	6	411595	7	NULL	NULL	0	NULL	PS I	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible dissociation of LHC I as an early structural change in the PS I complex after DDC-induced photoinhibition of PS I is discussed .
	manualset3
159371	1	411596	7	NULL	NULL	0	NULL	etiological factors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible etiological factors are discussed emphasizing the role of heredity and it can be concluded that the endocrine constitution predisposing to epiphyseolysis be hereditary .
	manualset3
159372	2	411596	7	NULL	NULL	NULL	NULL	heredity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The possible etiological factors are discussed emphasizing the role of heredity and it can be concluded that the endocrine constitution predisposing to epiphyseolysis be hereditary .
	manualset3
159373	3	411596	7	NULL	NULL	NULL	NULL	endocrine constitution	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The possible etiological factors are discussed emphasizing the role of heredity and it can be concluded that the endocrine constitution predisposing to epiphyseolysis be hereditary .
	manualset3
159374	4	411596	7	NULL	NULL	0	NULL	epiphyseolysis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible etiological factors are discussed emphasizing the role of heredity and it can be concluded that the endocrine constitution predisposing to epiphyseolysis be hereditary .
	manualset3
160317	5	411596	7	NULL	NULL	0	NULL	 role 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible etiological factors are discussed emphasizing the role of heredity and it can be concluded that the endocrine constitution predisposing to epiphyseolysis be hereditary .
	manualset3
159375	1	411597	7	NULL	NULL	0	NULL	proPP biosynthetic precursor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible existence of a proPP biosynthetic precursor has been investigated by rat incisor organ culture and examination of the 32P and 14C labeled products .
	manualset3
159376	2	411597	7	NULL	NULL	0	NULL	rat incisor organ culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible existence of a proPP biosynthetic precursor has been investigated by rat incisor organ culture and examination of the 32P and 14C labeled products .
	manualset3
159377	3	411597	7	NULL	NULL	0	NULL	examination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible existence of a proPP biosynthetic precursor has been investigated by rat incisor organ culture and examination of the 32P and 14C labeled products .
	manualset3
159378	4	411597	7	NULL	NULL	0	NULL	32P labeled products	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible existence of a proPP biosynthetic precursor has been investigated by rat incisor organ culture and examination of the 32P and 14C labeled products .
	manualset3
159379	5	411597	7	NULL	NULL	0	NULL	14C labeled products	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible existence of a proPP biosynthetic precursor has been investigated by rat incisor organ culture and examination of the 32P and 14C labeled products .
	manualset3
159380	1	411598	7	NULL	NULL	0	NULL	neurochemical changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible involvement of these neurochemical changes in the clinical actions of neuroleptics characteristically requiring long-term medication , such as the production of persistent ( tardive ) dyskinesias as well as the antipsychotic effect , is discussed .
	manualset3
159381	2	411598	7	NULL	NULL	0	NULL	clinical actions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible involvement of these neurochemical changes in the clinical actions of neuroleptics characteristically requiring long-term medication , such as the production of persistent ( tardive ) dyskinesias as well as the antipsychotic effect , is discussed .
	manualset3
159382	3	411598	7	NULL	NULL	NULL	NULL	neuroleptics	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The possible involvement of these neurochemical changes in the clinical actions of neuroleptics characteristically requiring long-term medication , such as the production of persistent ( tardive ) dyskinesias as well as the antipsychotic effect , is discussed .
	manualset3
159383	4	411598	7	NULL	NULL	0	NULL	long-term medication	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible involvement of these neurochemical changes in the clinical actions of neuroleptics characteristically requiring long-term medication , such as the production of persistent ( tardive ) dyskinesias as well as the antipsychotic effect , is discussed .
	manualset3
159384	5	411598	7	NULL	NULL	NULL	NULL	 production 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The possible involvement of these neurochemical changes in the clinical actions of neuroleptics characteristically requiring long-term medication , such as the production of persistent ( tardive ) dyskinesias as well as the antipsychotic effect , is discussed .
	manualset3
159385	6	411598	7	NULL	NULL	0	NULL	( tardive ) dyskinesias 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible involvement of these neurochemical changes in the clinical actions of neuroleptics characteristically requiring long-term medication , such as the production of persistent ( tardive ) dyskinesias as well as the antipsychotic effect , is discussed .
	manualset3
159386	7	411598	7	NULL	NULL	0	NULL	antipsychotic effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible involvement of these neurochemical changes in the clinical actions of neuroleptics characteristically requiring long-term medication , such as the production of persistent ( tardive ) dyskinesias as well as the antipsychotic effect , is discussed .
	manualset3
160318	8	411598	7	NULL	NULL	0	NULL	involvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible involvement of these neurochemical changes in the clinical actions of neuroleptics characteristically requiring long-term medication , such as the production of persistent ( tardive ) dyskinesias as well as the antipsychotic effect , is discussed .
	manualset3
159387	1	411599	7	NULL	NULL	0	NULL	AMOEBIC DYSENTERY	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	AMOEBIC DYSENTERY : THE OUTBREAK IN CHICAGO .
	manualset3
159388	2	411599	7	NULL	NULL	0	NULL	OUTBREAK	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	AMOEBIC DYSENTERY : THE OUTBREAK IN CHICAGO .
	manualset3
159389	3	411599	7	NULL	NULL	0	NULL	CHICAGO	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	AMOEBIC DYSENTERY : THE OUTBREAK IN CHICAGO .
	manualset3
159390	1	411600	7	NULL	NULL	0	NULL	mechanism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible mechanism of this phenomenon is that protein fragments enter the circulation after thyroid cell damage induced by radiation .
	manualset3
159391	2	411600	7	NULL	NULL	NULL	NULL	phenomenon	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The possible mechanism of this phenomenon is that protein fragments enter the circulation after thyroid cell damage induced by radiation .
	manualset3
159392	3	411600	7	NULL	NULL	0	NULL	protein fragments	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible mechanism of this phenomenon is that protein fragments enter the circulation after thyroid cell damage induced by radiation .
	manualset3
159393	4	411600	7	NULL	NULL	0	NULL	circulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible mechanism of this phenomenon is that protein fragments enter the circulation after thyroid cell damage induced by radiation .
	manualset3
159394	5	411600	7	NULL	NULL	NULL	NULL	thyroid cell damage	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The possible mechanism of this phenomenon is that protein fragments enter the circulation after thyroid cell damage induced by radiation .
	manualset3
159395	6	411600	7	NULL	NULL	0	NULL	 radiation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible mechanism of this phenomenon is that protein fragments enter the circulation after thyroid cell damage induced by radiation .
	manualset3
159396	1	411601	7	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible role of blisters in dermal burns .
	manualset3
159397	2	411601	7	NULL	NULL	0	NULL	blisters	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible role of blisters in dermal burns .
	manualset3
159398	3	411601	7	NULL	NULL	0	NULL	dermal burns 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible role of blisters in dermal burns .
	manualset3
159412	1	411602	7	NULL	NULL	NULL	NULL	role	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The possible role of interleukin-6 in the pathogenesis of the Crow-Fukase syndrome and the utility of DFPP treatment are discussed .
	manualset3
159413	2	411602	7	NULL	NULL	0	NULL	 interleukin-6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible role of interleukin-6 in the pathogenesis of the Crow-Fukase syndrome and the utility of DFPP treatment are discussed .
	manualset3
159414	3	411602	7	NULL	NULL	NULL	NULL	pathogenesis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The possible role of interleukin-6 in the pathogenesis of the Crow-Fukase syndrome and the utility of DFPP treatment are discussed .
	manualset3
159415	4	411602	7	NULL	NULL	0	NULL	Crow-Fukase syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible role of interleukin-6 in the pathogenesis of the Crow-Fukase syndrome and the utility of DFPP treatment are discussed .
	manualset3
159416	5	411602	7	NULL	NULL	0	NULL	DFPP treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible role of interleukin-6 in the pathogenesis of the Crow-Fukase syndrome and the utility of DFPP treatment are discussed .
	manualset3
159417	1	411603	7	NULL	NULL	NULL	NULL	 roles 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The possible roles of intracellular Ca2 + and protein kinase C in placental steroidogenesis are discussed .
	manualset3
159418	2	411603	7	NULL	NULL	0	NULL	intracellular Ca2 + 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible roles of intracellular Ca2 + and protein kinase C in placental steroidogenesis are discussed .
	manualset3
159419	3	411603	7	NULL	NULL	0	NULL	protein kinase C	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible roles of intracellular Ca2 + and protein kinase C in placental steroidogenesis are discussed .
	manualset3
159420	4	411603	7	NULL	NULL	0	NULL	 placental steroidogenesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible roles of intracellular Ca2 + and protein kinase C in placental steroidogenesis are discussed .
	manualset3
159421	1	411604	7	NULL	NULL	0	NULL	polytetrafluoroethylene ( Fluon ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible use of polytetrafluoroethylene ( Fluon ) as a tablet lubricant .
	manualset3
159422	2	411604	7	NULL	NULL	0	NULL	tablet lubricant	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible use of polytetrafluoroethylene ( Fluon ) as a tablet lubricant .
	manualset3
162700	3	411604	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The possible use of polytetrafluoroethylene ( Fluon ) as a tablet lubricant .
	manualset3
159423	1	411605	7	NULL	NULL	0	NULL	post-operative antalgic treatment protocol	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The post-operative antalgic treatment protocol included the random distribution of patients to three groups : control group : endovenous analgesia with morphine boluses ; group 1 : intrapleural analgesia with bupivacaine boluses ; group 2 : caudal epidural analgesia in a single bolus with a mix of bupivacaine and morphine .
	manualset3
159424	2	411605	7	NULL	NULL	0	NULL	random distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The post-operative antalgic treatment protocol included the random distribution of patients to three groups : control group : endovenous analgesia with morphine boluses ; group 1 : intrapleural analgesia with bupivacaine boluses ; group 2 : caudal epidural analgesia in a single bolus with a mix of bupivacaine and morphine .
	manualset3
159425	3	411605	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The post-operative antalgic treatment protocol included the random distribution of patients to three groups : control group : endovenous analgesia with morphine boluses ; group 1 : intrapleural analgesia with bupivacaine boluses ; group 2 : caudal epidural analgesia in a single bolus with a mix of bupivacaine and morphine .
	manualset3
159426	4	411605	7	NULL	NULL	0	NULL	three groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The post-operative antalgic treatment protocol included the random distribution of patients to three groups : control group : endovenous analgesia with morphine boluses ; group 1 : intrapleural analgesia with bupivacaine boluses ; group 2 : caudal epidural analgesia in a single bolus with a mix of bupivacaine and morphine .
	manualset3
159427	5	411605	7	NULL	NULL	0	NULL	control group 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The post-operative antalgic treatment protocol included the random distribution of patients to three groups : control group : endovenous analgesia with morphine boluses ; group 1 : intrapleural analgesia with bupivacaine boluses ; group 2 : caudal epidural analgesia in a single bolus with a mix of bupivacaine and morphine .
	manualset3
159428	6	411605	7	NULL	NULL	0	NULL	endovenous analgesia	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The post-operative antalgic treatment protocol included the random distribution of patients to three groups : control group : endovenous analgesia with morphine boluses ; group 1 : intrapleural analgesia with bupivacaine boluses ; group 2 : caudal epidural analgesia in a single bolus with a mix of bupivacaine and morphine .
	manualset3
159429	7	411605	7	NULL	NULL	0	NULL	morphine boluses	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The post-operative antalgic treatment protocol included the random distribution of patients to three groups : control group : endovenous analgesia with morphine boluses ; group 1 : intrapleural analgesia with bupivacaine boluses ; group 2 : caudal epidural analgesia in a single bolus with a mix of bupivacaine and morphine .
	manualset3
159430	8	411605	7	NULL	NULL	0	NULL	group 1	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The post-operative antalgic treatment protocol included the random distribution of patients to three groups : control group : endovenous analgesia with morphine boluses ; group 1 : intrapleural analgesia with bupivacaine boluses ; group 2 : caudal epidural analgesia in a single bolus with a mix of bupivacaine and morphine .
	manualset3
159431	9	411605	7	NULL	NULL	0	NULL	intrapleural analgesia	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The post-operative antalgic treatment protocol included the random distribution of patients to three groups : control group : endovenous analgesia with morphine boluses ; group 1 : intrapleural analgesia with bupivacaine boluses ; group 2 : caudal epidural analgesia in a single bolus with a mix of bupivacaine and morphine .
	manualset3
159432	10	411605	7	NULL	NULL	0	NULL	bupivacaine boluses	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The post-operative antalgic treatment protocol included the random distribution of patients to three groups : control group : endovenous analgesia with morphine boluses ; group 1 : intrapleural analgesia with bupivacaine boluses ; group 2 : caudal epidural analgesia in a single bolus with a mix of bupivacaine and morphine .
	manualset3
159433	11	411605	7	NULL	NULL	0	NULL	 group 2	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The post-operative antalgic treatment protocol included the random distribution of patients to three groups : control group : endovenous analgesia with morphine boluses ; group 1 : intrapleural analgesia with bupivacaine boluses ; group 2 : caudal epidural analgesia in a single bolus with a mix of bupivacaine and morphine .
	manualset3
159434	12	411605	7	NULL	NULL	0	NULL	caudal epidural analgesia 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The post-operative antalgic treatment protocol included the random distribution of patients to three groups : control group : endovenous analgesia with morphine boluses ; group 1 : intrapleural analgesia with bupivacaine boluses ; group 2 : caudal epidural analgesia in a single bolus with a mix of bupivacaine and morphine .
	manualset3
159435	13	411605	7	NULL	NULL	0	NULL	single bolus	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The post-operative antalgic treatment protocol included the random distribution of patients to three groups : control group : endovenous analgesia with morphine boluses ; group 1 : intrapleural analgesia with bupivacaine boluses ; group 2 : caudal epidural analgesia in a single bolus with a mix of bupivacaine and morphine .
	manualset3
159436	14	411605	7	NULL	NULL	0	NULL	bupivacaine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The post-operative antalgic treatment protocol included the random distribution of patients to three groups : control group : endovenous analgesia with morphine boluses ; group 1 : intrapleural analgesia with bupivacaine boluses ; group 2 : caudal epidural analgesia in a single bolus with a mix of bupivacaine and morphine .
	manualset3
159437	15	411605	7	NULL	NULL	0	NULL	morphine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The post-operative antalgic treatment protocol included the random distribution of patients to three groups : control group : endovenous analgesia with morphine boluses ; group 1 : intrapleural analgesia with bupivacaine boluses ; group 2 : caudal epidural analgesia in a single bolus with a mix of bupivacaine and morphine .
	manualset3
159438	1	411606	7	NULL	NULL	0	NULL	post-trial injection 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The post-trial injection of 1 ng SP ( in 0.5 microliter volume ) led to significantly longer latencies in the uphill response .
	manualset3
159439	2	411606	7	NULL	NULL	0	NULL	1 ng SP ( in 0.5 microliter volume )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The post-trial injection of 1 ng SP ( in 0.5 microliter volume ) led to significantly longer latencies in the uphill response .
	manualset3
159440	3	411606	7	NULL	NULL	0	NULL	 longer latencies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The post-trial injection of 1 ng SP ( in 0.5 microliter volume ) led to significantly longer latencies in the uphill response .
	manualset3
159441	4	411606	7	NULL	NULL	0	NULL	uphill response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The post-trial injection of 1 ng SP ( in 0.5 microliter volume ) led to significantly longer latencies in the uphill response .
	manualset3
159442	1	411607	7	NULL	NULL	0	NULL	AMP-dependence	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	AMP-dependence of the cyanide-insensitive pathway in the respiratory chain of Paramecium tetraurelia .
	manualset3
159443	2	411607	7	NULL	NULL	0	NULL	cyanide-insensitive pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	AMP-dependence of the cyanide-insensitive pathway in the respiratory chain of Paramecium tetraurelia .
	manualset3
159444	3	411607	7	NULL	NULL	NULL	NULL	respiratory chain	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	AMP-dependence of the cyanide-insensitive pathway in the respiratory chain of Paramecium tetraurelia .
	manualset3
159445	4	411607	7	NULL	NULL	0	NULL	Paramecium tetraurelia	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	AMP-dependence of the cyanide-insensitive pathway in the respiratory chain of Paramecium tetraurelia .
	manualset3
159446	1	411608	7	NULL	NULL	NULL	NULL	postmortem addition	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The postmortem addition of vitamin E ( OIL + E ) was slightly effective in retarding the oxidation of pigment and lipid , especially compared with the OIL treatments .
	manualset3
159448	3	411608	7	NULL	NULL	0	NULL	vitamin E ( OIL + E )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The postmortem addition of vitamin E ( OIL + E ) was slightly effective in retarding the oxidation of pigment and lipid , especially compared with the OIL treatments .
	manualset3
159449	4	411608	7	NULL	NULL	NULL	NULL	 oxidation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The postmortem addition of vitamin E ( OIL + E ) was slightly effective in retarding the oxidation of pigment and lipid , especially compared with the OIL treatments .
	manualset3
159450	5	411608	7	NULL	NULL	0	NULL	pigment	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The postmortem addition of vitamin E ( OIL + E ) was slightly effective in retarding the oxidation of pigment and lipid , especially compared with the OIL treatments .
	manualset3
159451	6	411608	7	NULL	NULL	0	NULL	lipid	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The postmortem addition of vitamin E ( OIL + E ) was slightly effective in retarding the oxidation of pigment and lipid , especially compared with the OIL treatments .
	manualset3
159452	7	411608	7	NULL	NULL	0	NULL	 OIL treatments	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The postmortem addition of vitamin E ( OIL + E ) was slightly effective in retarding the oxidation of pigment and lipid , especially compared with the OIL treatments .
	manualset3
159453	1	411609	7	NULL	NULL	0	NULL	postnatal weight pattern	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The postnatal weight pattern up to 14 weeks after birth was determined in 184 singleton survivors born at 23 to 29 weeks ' gestation in whom routine parenteral nutrition was used before milk feeding was established .
	manualset3
159454	2	411609	7	NULL	NULL	0	NULL	14 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The postnatal weight pattern up to 14 weeks after birth was determined in 184 singleton survivors born at 23 to 29 weeks ' gestation in whom routine parenteral nutrition was used before milk feeding was established .
	manualset3
159455	3	411609	7	NULL	NULL	0	NULL	birth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The postnatal weight pattern up to 14 weeks after birth was determined in 184 singleton survivors born at 23 to 29 weeks ' gestation in whom routine parenteral nutrition was used before milk feeding was established .
	manualset3
159456	4	411609	7	NULL	NULL	NULL	NULL	184 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The postnatal weight pattern up to 14 weeks after birth was determined in 184 singleton survivors born at 23 to 29 weeks ' gestation in whom routine parenteral nutrition was used before milk feeding was established .
	manualset3
159457	5	411609	7	NULL	NULL	0	NULL	23 to 29 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The postnatal weight pattern up to 14 weeks after birth was determined in 184 singleton survivors born at 23 to 29 weeks ' gestation in whom routine parenteral nutrition was used before milk feeding was established .
	manualset3
159458	6	411609	7	NULL	NULL	0	NULL	gestation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The postnatal weight pattern up to 14 weeks after birth was determined in 184 singleton survivors born at 23 to 29 weeks ' gestation in whom routine parenteral nutrition was used before milk feeding was established .
	manualset3
159459	7	411609	7	NULL	NULL	0	NULL	parenteral nutrition	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The postnatal weight pattern up to 14 weeks after birth was determined in 184 singleton survivors born at 23 to 29 weeks ' gestation in whom routine parenteral nutrition was used before milk feeding was established .
	manualset3
159460	8	411609	7	NULL	NULL	0	NULL	milk feeding 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The postnatal weight pattern up to 14 weeks after birth was determined in 184 singleton survivors born at 23 to 29 weeks ' gestation in whom routine parenteral nutrition was used before milk feeding was established .
	manualset3
159461	9	411609	7	NULL	NULL	0	NULL	singleton survivors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The postnatal weight pattern up to 14 weeks after birth was determined in 184 singleton survivors born at 23 to 29 weeks ' gestation in whom routine parenteral nutrition was used before milk feeding was established .
	manualset3
159462	1	411610	7	NULL	NULL	0	NULL	postoperative air-bone gap	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The postoperative air-bone gap in the 15 patients who were treated by ISRO with bone cement only excluding the 2 reoperation cases was 12.1 dB HL .
	manualset3
159463	2	411610	7	NULL	NULL	0	NULL	15 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The postoperative air-bone gap in the 15 patients who were treated by ISRO with bone cement only excluding the 2 reoperation cases was 12.1 dB HL .
	manualset3
159464	3	411610	7	NULL	NULL	0	NULL	ISRO	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The postoperative air-bone gap in the 15 patients who were treated by ISRO with bone cement only excluding the 2 reoperation cases was 12.1 dB HL .
	manualset3
159465	4	411610	7	NULL	NULL	0	NULL	bone cement	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The postoperative air-bone gap in the 15 patients who were treated by ISRO with bone cement only excluding the 2 reoperation cases was 12.1 dB HL .
	manualset3
159466	5	411610	7	NULL	NULL	0	NULL	2 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The postoperative air-bone gap in the 15 patients who were treated by ISRO with bone cement only excluding the 2 reoperation cases was 12.1 dB HL .
	manualset3
159467	6	411610	7	NULL	NULL	0	NULL	reoperation cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The postoperative air-bone gap in the 15 patients who were treated by ISRO with bone cement only excluding the 2 reoperation cases was 12.1 dB HL .
	manualset3
159468	7	411610	7	NULL	NULL	0	NULL	12.1 dB HL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The postoperative air-bone gap in the 15 patients who were treated by ISRO with bone cement only excluding the 2 reoperation cases was 12.1 dB HL .
	manualset3
159469	1	411611	7	NULL	NULL	0	NULL	 potential beneficial effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential beneficial effects of venom components are under investigation .
	manualset3
159470	2	411611	7	NULL	NULL	NULL	NULL	venom components	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The potential beneficial effects of venom components are under investigation .
	manualset3
159471	3	411611	7	NULL	NULL	0	NULL	 investigation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential beneficial effects of venom components are under investigation .
	manualset3
159472	1	411612	7	NULL	NULL	0	NULL	potential developmental and physical adverse effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential developmental and physical adverse effects these chronic pesticide exposures have on children are of increasing concern .
	manualset3
159473	2	411612	7	NULL	NULL	NULL	NULL	chronic pesticide  exposures	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The potential developmental and physical adverse effects these chronic pesticide exposures have on children are of increasing concern .
	manualset3
159474	3	411612	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential developmental and physical adverse effects these chronic pesticide exposures have on children are of increasing concern .
	manualset3
159475	1	411613	7	NULL	NULL	NULL	NULL	ADJUSTABLE DROP-CONTROL	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	AN ADJUSTABLE DROP-CONTROL FOR BURETTES .
	manualset3
159476	2	411613	7	NULL	NULL	NULL	NULL	BURETTES	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	AN ADJUSTABLE DROP-CONTROL FOR BURETTES .
	manualset3
159477	1	411614	7	NULL	NULL	0	NULL	potential effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential effect of vision loss on adolescents ' self-perception has been the subject of limited research .
	manualset3
159478	2	411614	7	NULL	NULL	0	NULL	vision loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential effect of vision loss on adolescents ' self-perception has been the subject of limited research .
	manualset3
159479	3	411614	7	NULL	NULL	0	NULL	adolescents ' self-perception	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential effect of vision loss on adolescents ' self-perception has been the subject of limited research .
	manualset3
159480	4	411614	7	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential effect of vision loss on adolescents ' self-perception has been the subject of limited research .
	manualset3
160319	5	411614	7	NULL	NULL	0	NULL	subject	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential effect of vision loss on adolescents ' self-perception has been the subject of limited research .
	manualset3
159481	1	411615	7	NULL	NULL	0	NULL	potential effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential effect was monitored by direct amplification , cloning and sequencing of bacterial DNA encoding 16S rRNA , and high-throughput DNA pyrosequencing of the bacterial DNA coding for the 16S rRNA hypervariable V6 region from bacterial communities grown in the two different media .
	manualset3
159482	2	411615	7	NULL	NULL	0	NULL	direct amplification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential effect was monitored by direct amplification , cloning and sequencing of bacterial DNA encoding 16S rRNA , and high-throughput DNA pyrosequencing of the bacterial DNA coding for the 16S rRNA hypervariable V6 region from bacterial communities grown in the two different media .
	manualset3
159483	3	411615	7	NULL	NULL	NULL	NULL	cloning 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The potential effect was monitored by direct amplification , cloning and sequencing of bacterial DNA encoding 16S rRNA , and high-throughput DNA pyrosequencing of the bacterial DNA coding for the 16S rRNA hypervariable V6 region from bacterial communities grown in the two different media .
	manualset3
159484	4	411615	7	NULL	NULL	NULL	NULL	bacterial DNA 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The potential effect was monitored by direct amplification , cloning and sequencing of bacterial DNA encoding 16S rRNA , and high-throughput DNA pyrosequencing of the bacterial DNA coding for the 16S rRNA hypervariable V6 region from bacterial communities grown in the two different media .
	manualset3
159485	5	411615	7	NULL	NULL	0	NULL	high-throughput DNA pyrosequencing 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential effect was monitored by direct amplification , cloning and sequencing of bacterial DNA encoding 16S rRNA , and high-throughput DNA pyrosequencing of the bacterial DNA coding for the 16S rRNA hypervariable V6 region from bacterial communities grown in the two different media .
	manualset3
159486	6	411615	7	NULL	NULL	0	NULL	 bacterial DNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential effect was monitored by direct amplification , cloning and sequencing of bacterial DNA encoding 16S rRNA , and high-throughput DNA pyrosequencing of the bacterial DNA coding for the 16S rRNA hypervariable V6 region from bacterial communities grown in the two different media .
	manualset3
159487	7	411615	7	NULL	NULL	0	NULL	16S rRNA hypervariable V6 region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential effect was monitored by direct amplification , cloning and sequencing of bacterial DNA encoding 16S rRNA , and high-throughput DNA pyrosequencing of the bacterial DNA coding for the 16S rRNA hypervariable V6 region from bacterial communities grown in the two different media .
	manualset3
159488	8	411615	7	NULL	NULL	0	NULL	bacterial communities	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential effect was monitored by direct amplification , cloning and sequencing of bacterial DNA encoding 16S rRNA , and high-throughput DNA pyrosequencing of the bacterial DNA coding for the 16S rRNA hypervariable V6 region from bacterial communities grown in the two different media .
	manualset3
159489	9	411615	7	NULL	NULL	0	NULL	two	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential effect was monitored by direct amplification , cloning and sequencing of bacterial DNA encoding 16S rRNA , and high-throughput DNA pyrosequencing of the bacterial DNA coding for the 16S rRNA hypervariable V6 region from bacterial communities grown in the two different media .
	manualset3
159490	10	411615	7	NULL	NULL	0	NULL	media	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential effect was monitored by direct amplification , cloning and sequencing of bacterial DNA encoding 16S rRNA , and high-throughput DNA pyrosequencing of the bacterial DNA coding for the 16S rRNA hypervariable V6 region from bacterial communities grown in the two different media .
	manualset3
159491	11	411615	7	NULL	NULL	0	NULL	16S rRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential effect was monitored by direct amplification , cloning and sequencing of bacterial DNA encoding 16S rRNA , and high-throughput DNA pyrosequencing of the bacterial DNA coding for the 16S rRNA hypervariable V6 region from bacterial communities grown in the two different media .
	manualset3
162701	12	411615	7	NULL	NULL	0	NULL	 sequencing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential effect was monitored by direct amplification , cloning and sequencing of bacterial DNA encoding 16S rRNA , and high-throughput DNA pyrosequencing of the bacterial DNA coding for the 16S rRNA hypervariable V6 region from bacterial communities grown in the two different media .
	manualset3
159492	1	411616	7	NULL	NULL	NULL	NULL	 potential impact 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The potential impact of Nutlin-3 on DNA repair in tumors suggests that Mdm2 inhibitors may significantly accentuate the tumoricidal actions of certain therapeutic modalities .
	manualset3
159493	2	411616	7	NULL	NULL	0	NULL	Nutlin-3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential impact of Nutlin-3 on DNA repair in tumors suggests that Mdm2 inhibitors may significantly accentuate the tumoricidal actions of certain therapeutic modalities .
	manualset3
159494	3	411616	7	NULL	NULL	0	NULL	DNA repair 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential impact of Nutlin-3 on DNA repair in tumors suggests that Mdm2 inhibitors may significantly accentuate the tumoricidal actions of certain therapeutic modalities .
	manualset3
159495	4	411616	7	NULL	NULL	0	NULL	tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential impact of Nutlin-3 on DNA repair in tumors suggests that Mdm2 inhibitors may significantly accentuate the tumoricidal actions of certain therapeutic modalities .
	manualset3
159496	5	411616	7	NULL	NULL	0	NULL	Mdm2 inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential impact of Nutlin-3 on DNA repair in tumors suggests that Mdm2 inhibitors may significantly accentuate the tumoricidal actions of certain therapeutic modalities .
	manualset3
159497	6	411616	7	NULL	NULL	0	NULL	tumoricidal actions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential impact of Nutlin-3 on DNA repair in tumors suggests that Mdm2 inhibitors may significantly accentuate the tumoricidal actions of certain therapeutic modalities .
	manualset3
159498	7	411616	7	NULL	NULL	0	NULL	therapeutic modalities	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential impact of Nutlin-3 on DNA repair in tumors suggests that Mdm2 inhibitors may significantly accentuate the tumoricidal actions of certain therapeutic modalities .
	manualset3
159499	1	411617	7	NULL	NULL	0	NULL	potential impact 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential impact of exenatide on morbidity and mortality is not known .
	manualset3
159500	2	411617	7	NULL	NULL	0	NULL	exenatide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential impact of exenatide on morbidity and mortality is not known .
	manualset3
159501	3	411617	7	NULL	NULL	NULL	NULL	morbidity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The potential impact of exenatide on morbidity and mortality is not known .
	manualset3
159502	4	411617	7	NULL	NULL	NULL	NULL	mortality	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The potential impact of exenatide on morbidity and mortality is not known .
	manualset3
159503	1	411618	7	NULL	NULL	0	NULL	 potential implication	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential implication of these observations in site-specific delivery of drug carriers is discussed .
	manualset3
159504	2	411618	7	NULL	NULL	0	NULL	observations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential implication of these observations in site-specific delivery of drug carriers is discussed .
	manualset3
159505	3	411618	7	NULL	NULL	0	NULL	site-specific delivery 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential implication of these observations in site-specific delivery of drug carriers is discussed .
	manualset3
159506	4	411618	7	NULL	NULL	0	NULL	drug carriers	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential implication of these observations in site-specific delivery of drug carriers is discussed .
	manualset3
159507	2	411619	7	NULL	NULL	NULL	NULL	 1-trichloromethyl-1 , 2 , 3 , 4 - tetrahydro-beta-carboline ( TaClo )	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The potential neurotoxin 1-trichloromethyl-1 , 2 , 3 , 4 - tetrahydro-beta-carboline ( TaClo ) has recently been suggested to be a causative factor in the clinical development of Parkinsonian symptoms after long-term exposure to precursor compounds such as the hypnotic chloral hydrate .
	manualset3
159508	1	411619	7	NULL	NULL	0	NULL	neurotoxin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential neurotoxin 1-trichloromethyl-1 , 2 , 3 , 4 - tetrahydro-beta-carboline ( TaClo ) has recently been suggested to be a causative factor in the clinical development of Parkinsonian symptoms after long-term exposure to precursor compounds such as the hypnotic chloral hydrate .
	manualset3
159509	3	411619	7	NULL	NULL	0	NULL	causative factor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential neurotoxin 1-trichloromethyl-1 , 2 , 3 , 4 - tetrahydro-beta-carboline ( TaClo ) has recently been suggested to be a causative factor in the clinical development of Parkinsonian symptoms after long-term exposure to precursor compounds such as the hypnotic chloral hydrate .
	manualset3
159510	4	411619	7	NULL	NULL	0	NULL	clinical development 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential neurotoxin 1-trichloromethyl-1 , 2 , 3 , 4 - tetrahydro-beta-carboline ( TaClo ) has recently been suggested to be a causative factor in the clinical development of Parkinsonian symptoms after long-term exposure to precursor compounds such as the hypnotic chloral hydrate .
	manualset3
159511	5	411619	7	NULL	NULL	0	NULL	Parkinsonian symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential neurotoxin 1-trichloromethyl-1 , 2 , 3 , 4 - tetrahydro-beta-carboline ( TaClo ) has recently been suggested to be a causative factor in the clinical development of Parkinsonian symptoms after long-term exposure to precursor compounds such as the hypnotic chloral hydrate .
	manualset3
159512	7	411619	7	NULL	NULL	NULL	NULL	precursor compounds	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The potential neurotoxin 1-trichloromethyl-1 , 2 , 3 , 4 - tetrahydro-beta-carboline ( TaClo ) has recently been suggested to be a causative factor in the clinical development of Parkinsonian symptoms after long-term exposure to precursor compounds such as the hypnotic chloral hydrate .
	manualset3
159513	8	411619	7	NULL	NULL	NULL	NULL	hypnotic chloral hydrate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The potential neurotoxin 1-trichloromethyl-1 , 2 , 3 , 4 - tetrahydro-beta-carboline ( TaClo ) has recently been suggested to be a causative factor in the clinical development of Parkinsonian symptoms after long-term exposure to precursor compounds such as the hypnotic chloral hydrate .
	manualset3
159514	6	411619	7	NULL	NULL	NULL	NULL	long-term exposure	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The potential neurotoxin 1-trichloromethyl-1 , 2 , 3 , 4 - tetrahydro-beta-carboline ( TaClo ) has recently been suggested to be a causative factor in the clinical development of Parkinsonian symptoms after long-term exposure to precursor compounds such as the hypnotic chloral hydrate .
	manualset3
159515	2	411620	7	NULL	NULL	NULL	NULL	education	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The potential protective role of education for dementia is an area of major interest .
	manualset3
159516	3	411620	7	NULL	NULL	NULL	NULL	 dementia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The potential protective role of education for dementia is an area of major interest .
	manualset3
159517	1	411620	7	NULL	NULL	NULL	NULL	 protective role	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The potential protective role of education for dementia is an area of major interest .
	manualset3
159518	4	411620	7	NULL	NULL	0	NULL	major interest	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential protective role of education for dementia is an area of major interest .
	manualset3
159519	1	411621	7	NULL	NULL	NULL	NULL	potential risk factors	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The potential risk factors of mortality and functional outcomes considered were ; ( 1 ) age , gender , body mass index , previous fracture history , preoperative ambulatory ability and residency type ; ( 2 ) 8 comorbidity items , cognitive impairment , smoking , and American Society of Anesthesiologists ' classification ; and ( 3 ) delay prior to surgery , fracture type , operation time , operation method , and postoperative fall history .
	manualset3
159520	2	411621	7	NULL	NULL	NULL	NULL	mortality	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The potential risk factors of mortality and functional outcomes considered were ; ( 1 ) age , gender , body mass index , previous fracture history , preoperative ambulatory ability and residency type ; ( 2 ) 8 comorbidity items , cognitive impairment , smoking , and American Society of Anesthesiologists ' classification ; and ( 3 ) delay prior to surgery , fracture type , operation time , operation method , and postoperative fall history .
	manualset3
159521	3	411621	7	NULL	NULL	0	NULL	 functional outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential risk factors of mortality and functional outcomes considered were ; ( 1 ) age , gender , body mass index , previous fracture history , preoperative ambulatory ability and residency type ; ( 2 ) 8 comorbidity items , cognitive impairment , smoking , and American Society of Anesthesiologists ' classification ; and ( 3 ) delay prior to surgery , fracture type , operation time , operation method , and postoperative fall history .
	manualset3
159522	4	411621	7	NULL	NULL	0	NULL	age 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential risk factors of mortality and functional outcomes considered were ; ( 1 ) age , gender , body mass index , previous fracture history , preoperative ambulatory ability and residency type ; ( 2 ) 8 comorbidity items , cognitive impairment , smoking , and American Society of Anesthesiologists ' classification ; and ( 3 ) delay prior to surgery , fracture type , operation time , operation method , and postoperative fall history .
	manualset3
159523	5	411621	7	NULL	NULL	0	NULL	 gender	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential risk factors of mortality and functional outcomes considered were ; ( 1 ) age , gender , body mass index , previous fracture history , preoperative ambulatory ability and residency type ; ( 2 ) 8 comorbidity items , cognitive impairment , smoking , and American Society of Anesthesiologists ' classification ; and ( 3 ) delay prior to surgery , fracture type , operation time , operation method , and postoperative fall history .
	manualset3
159524	6	411621	7	NULL	NULL	0	NULL	body mass index	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential risk factors of mortality and functional outcomes considered were ; ( 1 ) age , gender , body mass index , previous fracture history , preoperative ambulatory ability and residency type ; ( 2 ) 8 comorbidity items , cognitive impairment , smoking , and American Society of Anesthesiologists ' classification ; and ( 3 ) delay prior to surgery , fracture type , operation time , operation method , and postoperative fall history .
	manualset3
159525	7	411621	7	NULL	NULL	0	NULL	previous fracture history 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential risk factors of mortality and functional outcomes considered were ; ( 1 ) age , gender , body mass index , previous fracture history , preoperative ambulatory ability and residency type ; ( 2 ) 8 comorbidity items , cognitive impairment , smoking , and American Society of Anesthesiologists ' classification ; and ( 3 ) delay prior to surgery , fracture type , operation time , operation method , and postoperative fall history .
	manualset3
159526	8	411621	7	NULL	NULL	0	NULL	preoperative ambulatory ability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential risk factors of mortality and functional outcomes considered were ; ( 1 ) age , gender , body mass index , previous fracture history , preoperative ambulatory ability and residency type ; ( 2 ) 8 comorbidity items , cognitive impairment , smoking , and American Society of Anesthesiologists ' classification ; and ( 3 ) delay prior to surgery , fracture type , operation time , operation method , and postoperative fall history .
	manualset3
159527	9	411621	7	NULL	NULL	0	NULL	residency type	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential risk factors of mortality and functional outcomes considered were ; ( 1 ) age , gender , body mass index , previous fracture history , preoperative ambulatory ability and residency type ; ( 2 ) 8 comorbidity items , cognitive impairment , smoking , and American Society of Anesthesiologists ' classification ; and ( 3 ) delay prior to surgery , fracture type , operation time , operation method , and postoperative fall history .
	manualset3
159528	10	411621	7	NULL	NULL	0	NULL	comorbidity items	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential risk factors of mortality and functional outcomes considered were ; ( 1 ) age , gender , body mass index , previous fracture history , preoperative ambulatory ability and residency type ; ( 2 ) 8 comorbidity items , cognitive impairment , smoking , and American Society of Anesthesiologists ' classification ; and ( 3 ) delay prior to surgery , fracture type , operation time , operation method , and postoperative fall history .
	manualset3
159529	11	411621	7	NULL	NULL	0	NULL	cognitive impairment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential risk factors of mortality and functional outcomes considered were ; ( 1 ) age , gender , body mass index , previous fracture history , preoperative ambulatory ability and residency type ; ( 2 ) 8 comorbidity items , cognitive impairment , smoking , and American Society of Anesthesiologists ' classification ; and ( 3 ) delay prior to surgery , fracture type , operation time , operation method , and postoperative fall history .
	manualset3
159530	12	411621	7	NULL	NULL	0	NULL	smoking	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential risk factors of mortality and functional outcomes considered were ; ( 1 ) age , gender , body mass index , previous fracture history , preoperative ambulatory ability and residency type ; ( 2 ) 8 comorbidity items , cognitive impairment , smoking , and American Society of Anesthesiologists ' classification ; and ( 3 ) delay prior to surgery , fracture type , operation time , operation method , and postoperative fall history .
	manualset3
159531	13	411621	7	NULL	NULL	NULL	NULL	American Society of Anesthesiologists ' classification	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The potential risk factors of mortality and functional outcomes considered were ; ( 1 ) age , gender , body mass index , previous fracture history , preoperative ambulatory ability and residency type ; ( 2 ) 8 comorbidity items , cognitive impairment , smoking , and American Society of Anesthesiologists ' classification ; and ( 3 ) delay prior to surgery , fracture type , operation time , operation method , and postoperative fall history .
	manualset3
159532	14	411621	7	NULL	NULL	0	NULL	 delay prior to surgery	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential risk factors of mortality and functional outcomes considered were ; ( 1 ) age , gender , body mass index , previous fracture history , preoperative ambulatory ability and residency type ; ( 2 ) 8 comorbidity items , cognitive impairment , smoking , and American Society of Anesthesiologists ' classification ; and ( 3 ) delay prior to surgery , fracture type , operation time , operation method , and postoperative fall history .
	manualset3
159533	15	411621	7	NULL	NULL	0	NULL	fracture type	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential risk factors of mortality and functional outcomes considered were ; ( 1 ) age , gender , body mass index , previous fracture history , preoperative ambulatory ability and residency type ; ( 2 ) 8 comorbidity items , cognitive impairment , smoking , and American Society of Anesthesiologists ' classification ; and ( 3 ) delay prior to surgery , fracture type , operation time , operation method , and postoperative fall history .
	manualset3
159534	16	411621	7	NULL	NULL	0	NULL	operation time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential risk factors of mortality and functional outcomes considered were ; ( 1 ) age , gender , body mass index , previous fracture history , preoperative ambulatory ability and residency type ; ( 2 ) 8 comorbidity items , cognitive impairment , smoking , and American Society of Anesthesiologists ' classification ; and ( 3 ) delay prior to surgery , fracture type , operation time , operation method , and postoperative fall history .
	manualset3
159535	17	411621	7	NULL	NULL	0	NULL	operation method	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential risk factors of mortality and functional outcomes considered were ; ( 1 ) age , gender , body mass index , previous fracture history , preoperative ambulatory ability and residency type ; ( 2 ) 8 comorbidity items , cognitive impairment , smoking , and American Society of Anesthesiologists ' classification ; and ( 3 ) delay prior to surgery , fracture type , operation time , operation method , and postoperative fall history .
	manualset3
159536	18	411621	7	NULL	NULL	0	NULL	postoperative fall history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential risk factors of mortality and functional outcomes considered were ; ( 1 ) age , gender , body mass index , previous fracture history , preoperative ambulatory ability and residency type ; ( 2 ) 8 comorbidity items , cognitive impairment , smoking , and American Society of Anesthesiologists ' classification ; and ( 3 ) delay prior to surgery , fracture type , operation time , operation method , and postoperative fall history .
	manualset3
159537	1	411622	7	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential role of HCV in the pathogenesis of MPGN , which occurs in almost half of the cases of MC patients , has not been fully investigated , and the demonstration of HCV proteins as the antigenic constituent of the glomerular immune deposits has remained elusive .
	manualset3
159538	2	411622	7	NULL	NULL	0	NULL	HCV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential role of HCV in the pathogenesis of MPGN , which occurs in almost half of the cases of MC patients , has not been fully investigated , and the demonstration of HCV proteins as the antigenic constituent of the glomerular immune deposits has remained elusive .
	manualset3
159539	3	411622	7	NULL	NULL	0	NULL	pathogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential role of HCV in the pathogenesis of MPGN , which occurs in almost half of the cases of MC patients , has not been fully investigated , and the demonstration of HCV proteins as the antigenic constituent of the glomerular immune deposits has remained elusive .
	manualset3
159540	4	411622	7	NULL	NULL	0	NULL	MPGN	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential role of HCV in the pathogenesis of MPGN , which occurs in almost half of the cases of MC patients , has not been fully investigated , and the demonstration of HCV proteins as the antigenic constituent of the glomerular immune deposits has remained elusive .
	manualset3
159541	5	411622	7	NULL	NULL	0	NULL	MC patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential role of HCV in the pathogenesis of MPGN , which occurs in almost half of the cases of MC patients , has not been fully investigated , and the demonstration of HCV proteins as the antigenic constituent of the glomerular immune deposits has remained elusive .
	manualset3
159542	6	411622	7	NULL	NULL	0	NULL	demonstration	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential role of HCV in the pathogenesis of MPGN , which occurs in almost half of the cases of MC patients , has not been fully investigated , and the demonstration of HCV proteins as the antigenic constituent of the glomerular immune deposits has remained elusive .
	manualset3
159543	7	411622	7	NULL	NULL	NULL	NULL	HCV proteins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The potential role of HCV in the pathogenesis of MPGN , which occurs in almost half of the cases of MC patients , has not been fully investigated , and the demonstration of HCV proteins as the antigenic constituent of the glomerular immune deposits has remained elusive .
	manualset3
159544	8	411622	7	NULL	NULL	0	NULL	antigenic constituent	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential role of HCV in the pathogenesis of MPGN , which occurs in almost half of the cases of MC patients , has not been fully investigated , and the demonstration of HCV proteins as the antigenic constituent of the glomerular immune deposits has remained elusive .
	manualset3
159545	9	411622	7	NULL	NULL	0	NULL	glomerular immune deposits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential role of HCV in the pathogenesis of MPGN , which occurs in almost half of the cases of MC patients , has not been fully investigated , and the demonstration of HCV proteins as the antigenic constituent of the glomerular immune deposits has remained elusive .
	manualset3
162702	10	411622	7	NULL	NULL	0	NULL	cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential role of HCV in the pathogenesis of MPGN , which occurs in almost half of the cases of MC patients , has not been fully investigated , and the demonstration of HCV proteins as the antigenic constituent of the glomerular immune deposits has remained elusive .
	manualset3
159546	1	411623	7	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential role of vWf in leukocyte recruitment was investigated with the use of vWf-deficient mice .
	manualset3
159547	2	411623	7	NULL	NULL	0	NULL	 vWf	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential role of vWf in leukocyte recruitment was investigated with the use of vWf-deficient mice .
	manualset3
159548	3	411623	7	NULL	NULL	0	NULL	 leukocyte recruitment	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential role of vWf in leukocyte recruitment was investigated with the use of vWf-deficient mice .
	manualset3
159549	4	411623	7	NULL	NULL	0	NULL	vWf-deficient mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential role of vWf in leukocyte recruitment was investigated with the use of vWf-deficient mice .
	manualset3
159550	1	411624	7	NULL	NULL	0	NULL	 anticancer agent binding 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential for anticancer agent binding to cellulose nitrate/cellulose acetate and teflon membrane ultrafilters was documented , and quantitation of these anticancer agents based upon absorbance and fluorescence spectroscopy was performed .
	manualset3
159551	2	411624	7	NULL	NULL	0	NULL	cellulose nitrate/cellulose acetate ultrafilters 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential for anticancer agent binding to cellulose nitrate/cellulose acetate and teflon membrane ultrafilters was documented , and quantitation of these anticancer agents based upon absorbance and fluorescence spectroscopy was performed .
	manualset3
159552	3	411624	7	NULL	NULL	0	NULL	teflon membrane ultrafilters	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential for anticancer agent binding to cellulose nitrate/cellulose acetate and teflon membrane ultrafilters was documented , and quantitation of these anticancer agents based upon absorbance and fluorescence spectroscopy was performed .
	manualset3
159553	4	411624	7	NULL	NULL	0	NULL	quantitation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential for anticancer agent binding to cellulose nitrate/cellulose acetate and teflon membrane ultrafilters was documented , and quantitation of these anticancer agents based upon absorbance and fluorescence spectroscopy was performed .
	manualset3
159554	5	411624	7	NULL	NULL	0	NULL	anticancer agents 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential for anticancer agent binding to cellulose nitrate/cellulose acetate and teflon membrane ultrafilters was documented , and quantitation of these anticancer agents based upon absorbance and fluorescence spectroscopy was performed .
	manualset3
159555	6	411624	7	NULL	NULL	0	NULL	absorbance and fluorescence spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential for anticancer agent binding to cellulose nitrate/cellulose acetate and teflon membrane ultrafilters was documented , and quantitation of these anticancer agents based upon absorbance and fluorescence spectroscopy was performed .
	manualset3
162703	7	411624	7	NULL	NULL	0	NULL	potential 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential for anticancer agent binding to cellulose nitrate/cellulose acetate and teflon membrane ultrafilters was documented , and quantitation of these anticancer agents based upon absorbance and fluorescence spectroscopy was performed .
	manualset3
159556	1	411625	7	NULL	NULL	0	NULL	power spectral regime	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The power spectral regime above 200 cm ( -1 ) in all three systems is dominated by resonances due to localized vibrations , such as librations .
	manualset3
159557	2	411625	7	NULL	NULL	0	NULL	200 cm ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The power spectral regime above 200 cm ( -1 ) in all three systems is dominated by resonances due to localized vibrations , such as librations .
	manualset3
159558	3	411625	7	NULL	NULL	NULL	NULL	three systems	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The power spectral regime above 200 cm ( -1 ) in all three systems is dominated by resonances due to localized vibrations , such as librations .
	manualset3
159559	4	411625	7	NULL	NULL	NULL	NULL	resonances	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The power spectral regime above 200 cm ( -1 ) in all three systems is dominated by resonances due to localized vibrations , such as librations .
	manualset3
159560	5	411625	7	NULL	NULL	NULL	NULL	 localized vibrations	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The power spectral regime above 200 cm ( -1 ) in all three systems is dominated by resonances due to localized vibrations , such as librations .
	manualset3
159561	6	411625	7	NULL	NULL	NULL	NULL	 librations 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The power spectral regime above 200 cm ( -1 ) in all three systems is dominated by resonances due to localized vibrations , such as librations .
	manualset3
159562	1	411626	7	NULL	NULL	0	NULL	practical training 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The practical training will take place in centres with established medical obstetric clinics and will be tailored ( with appropriate modules ) to the amount of previous experience in medicine or obstetrics .
	manualset3
159563	2	411626	7	NULL	NULL	0	NULL	centres	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The practical training will take place in centres with established medical obstetric clinics and will be tailored ( with appropriate modules ) to the amount of previous experience in medicine or obstetrics .
	manualset3
159564	3	411626	7	NULL	NULL	0	NULL	medical obstetric clinics	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The practical training will take place in centres with established medical obstetric clinics and will be tailored ( with appropriate modules ) to the amount of previous experience in medicine or obstetrics .
	manualset3
159565	4	411626	7	NULL	NULL	NULL	NULL	modules	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The practical training will take place in centres with established medical obstetric clinics and will be tailored ( with appropriate modules ) to the amount of previous experience in medicine or obstetrics .
	manualset3
159566	5	411626	7	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The practical training will take place in centres with established medical obstetric clinics and will be tailored ( with appropriate modules ) to the amount of previous experience in medicine or obstetrics .
	manualset3
159567	6	411626	7	NULL	NULL	0	NULL	experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The practical training will take place in centres with established medical obstetric clinics and will be tailored ( with appropriate modules ) to the amount of previous experience in medicine or obstetrics .
	manualset3
159568	7	411626	7	NULL	NULL	0	NULL	 medicine	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The practical training will take place in centres with established medical obstetric clinics and will be tailored ( with appropriate modules ) to the amount of previous experience in medicine or obstetrics .
	manualset3
159569	8	411626	7	NULL	NULL	0	NULL	obstetrics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The practical training will take place in centres with established medical obstetric clinics and will be tailored ( with appropriate modules ) to the amount of previous experience in medicine or obstetrics .
	manualset3
159570	1	411627	7	NULL	NULL	0	NULL	 precontraction values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The precontraction values of glycogen , glucose and phosphocreatine were reduced .
	manualset3
159571	2	411627	7	NULL	NULL	0	NULL	 glycogen	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The precontraction values of glycogen , glucose and phosphocreatine were reduced .
	manualset3
159572	3	411627	7	NULL	NULL	0	NULL	glucose	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The precontraction values of glycogen , glucose and phosphocreatine were reduced .
	manualset3
159573	4	411627	7	NULL	NULL	0	NULL	phosphocreatine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The precontraction values of glycogen , glucose and phosphocreatine were reduced .
	manualset3
159574	1	411628	7	NULL	NULL	0	NULL	predialysis course	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The predialysis course includes a meeting among all those involved with the patient ( nephrologists , nurses , dieticians ) to exchange information with the purpose of shared evaluation and decision-making .
	manualset3
159575	2	411628	7	NULL	NULL	0	NULL	meeting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The predialysis course includes a meeting among all those involved with the patient ( nephrologists , nurses , dieticians ) to exchange information with the purpose of shared evaluation and decision-making .
	manualset3
159576	3	411628	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The predialysis course includes a meeting among all those involved with the patient ( nephrologists , nurses , dieticians ) to exchange information with the purpose of shared evaluation and decision-making .
	manualset3
159577	4	411628	7	NULL	NULL	0	NULL	nephrologists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The predialysis course includes a meeting among all those involved with the patient ( nephrologists , nurses , dieticians ) to exchange information with the purpose of shared evaluation and decision-making .
	manualset3
159578	5	411628	7	NULL	NULL	0	NULL	nurses	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The predialysis course includes a meeting among all those involved with the patient ( nephrologists , nurses , dieticians ) to exchange information with the purpose of shared evaluation and decision-making .
	manualset3
159579	6	411628	7	NULL	NULL	0	NULL	dieticians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The predialysis course includes a meeting among all those involved with the patient ( nephrologists , nurses , dieticians ) to exchange information with the purpose of shared evaluation and decision-making .
	manualset3
159580	7	411628	7	NULL	NULL	0	NULL	information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The predialysis course includes a meeting among all those involved with the patient ( nephrologists , nurses , dieticians ) to exchange information with the purpose of shared evaluation and decision-making .
	manualset3
159581	8	411628	7	NULL	NULL	0	NULL	 purpose	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The predialysis course includes a meeting among all those involved with the patient ( nephrologists , nurses , dieticians ) to exchange information with the purpose of shared evaluation and decision-making .
	manualset3
159582	9	411628	7	NULL	NULL	0	NULL	shared evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The predialysis course includes a meeting among all those involved with the patient ( nephrologists , nurses , dieticians ) to exchange information with the purpose of shared evaluation and decision-making .
	manualset3
159583	10	411628	7	NULL	NULL	0	NULL	decision-making	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The predialysis course includes a meeting among all those involved with the patient ( nephrologists , nurses , dieticians ) to exchange information with the purpose of shared evaluation and decision-making .
	manualset3
159584	1	411629	7	NULL	NULL	0	NULL	 predicted coding region 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The predicted coding region , which spans 543 amino acids , established the complete amino acid sequence of the L-type isozyme of pyruvate kinase for the first time .
	manualset3
159585	2	411629	7	NULL	NULL	0	NULL	543 amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The predicted coding region , which spans 543 amino acids , established the complete amino acid sequence of the L-type isozyme of pyruvate kinase for the first time .
	manualset3
159586	3	411629	7	NULL	NULL	0	NULL	complete amino acid sequence	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The predicted coding region , which spans 543 amino acids , established the complete amino acid sequence of the L-type isozyme of pyruvate kinase for the first time .
	manualset3
159588	4	411629	7	NULL	NULL	NULL	NULL	L-type isozyme of pyruvate kinase	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The predicted coding region , which spans 543 amino acids , established the complete amino acid sequence of the L-type isozyme of pyruvate kinase for the first time .
	manualset3
159589	6	411629	7	NULL	NULL	0	NULL	first time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The predicted coding region , which spans 543 amino acids , established the complete amino acid sequence of the L-type isozyme of pyruvate kinase for the first time .
	manualset3
159590	1	411630	7	NULL	NULL	0	NULL	predicted tertiary structure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The predicted tertiary structure of the native TRPS1 after refinement and validation was successfully submitted to the Protein Model Database and was assigned with PMDB ID PM0077843 , as it was previously unpredicted .
	manualset3
159591	2	411630	7	NULL	NULL	0	NULL	native TRPS1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The predicted tertiary structure of the native TRPS1 after refinement and validation was successfully submitted to the Protein Model Database and was assigned with PMDB ID PM0077843 , as it was previously unpredicted .
	manualset3
159592	3	411630	7	NULL	NULL	0	NULL	validation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The predicted tertiary structure of the native TRPS1 after refinement and validation was successfully submitted to the Protein Model Database and was assigned with PMDB ID PM0077843 , as it was previously unpredicted .
	manualset3
159593	4	411630	7	NULL	NULL	0	NULL	Protein Model Database	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The predicted tertiary structure of the native TRPS1 after refinement and validation was successfully submitted to the Protein Model Database and was assigned with PMDB ID PM0077843 , as it was previously unpredicted .
	manualset3
159594	5	411630	7	NULL	NULL	0	NULL	PMDB ID PM0077843 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The predicted tertiary structure of the native TRPS1 after refinement and validation was successfully submitted to the Protein Model Database and was assigned with PMDB ID PM0077843 , as it was previously unpredicted .
	manualset3
162704	6	411630	7	NULL	NULL	0	NULL	refinement	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The predicted tertiary structure of the native TRPS1 after refinement and validation was successfully submitted to the Protein Model Database and was assigned with PMDB ID PM0077843 , as it was previously unpredicted .
	manualset3
159595	1	411631	7	NULL	NULL	NULL	NULL	predicted three-dimension structure	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The predicted three-dimension structure of TaCAD1 resembled that of AtCAD5 , but two amino acid substitutions were identified in the substrate binding region .
	manualset3
159596	2	411631	7	NULL	NULL	0	NULL	TaCAD1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The predicted three-dimension structure of TaCAD1 resembled that of AtCAD5 , but two amino acid substitutions were identified in the substrate binding region .
	manualset3
159597	3	411631	7	NULL	NULL	0	NULL	AtCAD5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The predicted three-dimension structure of TaCAD1 resembled that of AtCAD5 , but two amino acid substitutions were identified in the substrate binding region .
	manualset3
159598	4	411631	7	NULL	NULL	NULL	NULL	two amino acid substitutions	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The predicted three-dimension structure of TaCAD1 resembled that of AtCAD5 , but two amino acid substitutions were identified in the substrate binding region .
	manualset3
159599	5	411631	7	NULL	NULL	0	NULL	substrate binding region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The predicted three-dimension structure of TaCAD1 resembled that of AtCAD5 , but two amino acid substitutions were identified in the substrate binding region .
	manualset3
159600	1	411632	7	NULL	NULL	0	NULL	predictors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The predictors of recurrent febrile seizures include younger age , lower threshold of temperature , onset within one hour of fever and positive family history .
	manualset3
159601	2	411632	7	NULL	NULL	0	NULL	recurrent febrile seizures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The predictors of recurrent febrile seizures include younger age , lower threshold of temperature , onset within one hour of fever and positive family history .
	manualset3
159602	3	411632	7	NULL	NULL	NULL	NULL	age	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The predictors of recurrent febrile seizures include younger age , lower threshold of temperature , onset within one hour of fever and positive family history .
	manualset3
159603	4	411632	7	NULL	NULL	NULL	NULL	 temperature	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The predictors of recurrent febrile seizures include younger age , lower threshold of temperature , onset within one hour of fever and positive family history .
	manualset3
159604	5	411632	7	NULL	NULL	0	NULL	onset within one hour of fever	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The predictors of recurrent febrile seizures include younger age , lower threshold of temperature , onset within one hour of fever and positive family history .
	manualset3
159605	6	411632	7	NULL	NULL	0	NULL	positive family history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The predictors of recurrent febrile seizures include younger age , lower threshold of temperature , onset within one hour of fever and positive family history .
	manualset3
159606	1	411633	7	NULL	NULL	NULL	NULL	G	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The predominant form of G produced by RSV-3 was found in infected cell supernatants , consistent with the size of secreted G .
	manualset3
159607	2	411633	7	NULL	NULL	0	NULL	RSV-3	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The predominant form of G produced by RSV-3 was found in infected cell supernatants , consistent with the size of secreted G .
	manualset3
159608	3	411633	7	NULL	NULL	NULL	NULL	cell supernatants	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The predominant form of G produced by RSV-3 was found in infected cell supernatants , consistent with the size of secreted G .
	manualset3
159609	4	411633	7	NULL	NULL	0	NULL	size 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The predominant form of G produced by RSV-3 was found in infected cell supernatants , consistent with the size of secreted G .
	manualset3
159610	5	411633	7	NULL	NULL	NULL	NULL	secreted G	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The predominant form of G produced by RSV-3 was found in infected cell supernatants , consistent with the size of secreted G .
	manualset3
159611	1	411634	7	NULL	NULL	0	NULL	organisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The predominant organisms isolated were Staphylococcus species , aerobic spore bearers , Klebsiella pneumoniae , Campylobacter jejuni , Acinetobacter species and Streptococcus species .
	manualset3
159612	2	411634	7	NULL	NULL	0	NULL	Staphylococcus species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The predominant organisms isolated were Staphylococcus species , aerobic spore bearers , Klebsiella pneumoniae , Campylobacter jejuni , Acinetobacter species and Streptococcus species .
	manualset3
159613	3	411634	7	NULL	NULL	0	NULL	aerobic spore bearers	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The predominant organisms isolated were Staphylococcus species , aerobic spore bearers , Klebsiella pneumoniae , Campylobacter jejuni , Acinetobacter species and Streptococcus species .
	manualset3
159614	4	411634	7	NULL	NULL	0	NULL	Klebsiella pneumoniae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The predominant organisms isolated were Staphylococcus species , aerobic spore bearers , Klebsiella pneumoniae , Campylobacter jejuni , Acinetobacter species and Streptococcus species .
	manualset3
159615	5	411634	7	NULL	NULL	0	NULL	Campylobacter jejuni	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The predominant organisms isolated were Staphylococcus species , aerobic spore bearers , Klebsiella pneumoniae , Campylobacter jejuni , Acinetobacter species and Streptococcus species .
	manualset3
159616	6	411634	7	NULL	NULL	0	NULL	Acinetobacter species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The predominant organisms isolated were Staphylococcus species , aerobic spore bearers , Klebsiella pneumoniae , Campylobacter jejuni , Acinetobacter species and Streptococcus species .
	manualset3
159617	7	411634	7	NULL	NULL	0	NULL	Streptococcus species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The predominant organisms isolated were Staphylococcus species , aerobic spore bearers , Klebsiella pneumoniae , Campylobacter jejuni , Acinetobacter species and Streptococcus species .
	manualset3
159618	1	411635	7	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The predominant role of adenosine triphosphate-sensitive K ( + ) current in switching on and off the repetitive firing of action potentials at 8 mM ( G ) was taken over at a higher ( G ) by Ca ( 2 + ) - or Na ( + ) - dependent currents , which were generated by the plasma membrane Ca ( 2 + ) pump , Na ( + ) / K ( + ) pump , Na ( + ) / Ca ( 2 + ) exchanger , and TRPM channel .
	manualset3
159619	2	411635	7	NULL	NULL	NULL	NULL	adenosine triphosphate-sensitive K ( + ) current	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The predominant role of adenosine triphosphate-sensitive K ( + ) current in switching on and off the repetitive firing of action potentials at 8 mM ( G ) was taken over at a higher ( G ) by Ca ( 2 + ) - or Na ( + ) - dependent currents , which were generated by the plasma membrane Ca ( 2 + ) pump , Na ( + ) / K ( + ) pump , Na ( + ) / Ca ( 2 + ) exchanger , and TRPM channel .
	manualset3
159620	3	411635	7	NULL	NULL	0	NULL	action potentials	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The predominant role of adenosine triphosphate-sensitive K ( + ) current in switching on and off the repetitive firing of action potentials at 8 mM ( G ) was taken over at a higher ( G ) by Ca ( 2 + ) - or Na ( + ) - dependent currents , which were generated by the plasma membrane Ca ( 2 + ) pump , Na ( + ) / K ( + ) pump , Na ( + ) / Ca ( 2 + ) exchanger , and TRPM channel .
	manualset3
159621	4	411635	7	NULL	NULL	0	NULL	8 mM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The predominant role of adenosine triphosphate-sensitive K ( + ) current in switching on and off the repetitive firing of action potentials at 8 mM ( G ) was taken over at a higher ( G ) by Ca ( 2 + ) - or Na ( + ) - dependent currents , which were generated by the plasma membrane Ca ( 2 + ) pump , Na ( + ) / K ( + ) pump , Na ( + ) / Ca ( 2 + ) exchanger , and TRPM channel .
	manualset3
159622	5	411635	7	NULL	NULL	NULL	NULL	Ca ( 2 + ) - dependent currents	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The predominant role of adenosine triphosphate-sensitive K ( + ) current in switching on and off the repetitive firing of action potentials at 8 mM ( G ) was taken over at a higher ( G ) by Ca ( 2 + ) - or Na ( + ) - dependent currents , which were generated by the plasma membrane Ca ( 2 + ) pump , Na ( + ) / K ( + ) pump , Na ( + ) / Ca ( 2 + ) exchanger , and TRPM channel .
	manualset3
159623	6	411635	7	NULL	NULL	0	NULL	plasma membrane Ca ( 2 + ) pump	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The predominant role of adenosine triphosphate-sensitive K ( + ) current in switching on and off the repetitive firing of action potentials at 8 mM ( G ) was taken over at a higher ( G ) by Ca ( 2 + ) - or Na ( + ) - dependent currents , which were generated by the plasma membrane Ca ( 2 + ) pump , Na ( + ) / K ( + ) pump , Na ( + ) / Ca ( 2 + ) exchanger , and TRPM channel .
	manualset3
159624	7	411635	7	NULL	NULL	0	NULL	Na ( + ) / K ( + ) pump	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The predominant role of adenosine triphosphate-sensitive K ( + ) current in switching on and off the repetitive firing of action potentials at 8 mM ( G ) was taken over at a higher ( G ) by Ca ( 2 + ) - or Na ( + ) - dependent currents , which were generated by the plasma membrane Ca ( 2 + ) pump , Na ( + ) / K ( + ) pump , Na ( + ) / Ca ( 2 + ) exchanger , and TRPM channel .
	manualset3
159625	8	411635	7	NULL	NULL	0	NULL	Na ( + ) / Ca ( 2 + ) exchanger	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The predominant role of adenosine triphosphate-sensitive K ( + ) current in switching on and off the repetitive firing of action potentials at 8 mM ( G ) was taken over at a higher ( G ) by Ca ( 2 + ) - or Na ( + ) - dependent currents , which were generated by the plasma membrane Ca ( 2 + ) pump , Na ( + ) / K ( + ) pump , Na ( + ) / Ca ( 2 + ) exchanger , and TRPM channel .
	manualset3
159626	9	411635	7	NULL	NULL	0	NULL	TRPM channel	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The predominant role of adenosine triphosphate-sensitive K ( + ) current in switching on and off the repetitive firing of action potentials at 8 mM ( G ) was taken over at a higher ( G ) by Ca ( 2 + ) - or Na ( + ) - dependent currents , which were generated by the plasma membrane Ca ( 2 + ) pump , Na ( + ) / K ( + ) pump , Na ( + ) / Ca ( 2 + ) exchanger , and TRPM channel .
	manualset3
159627	10	411635	7	NULL	NULL	NULL	NULL	Na ( + ) - dependent currents	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The predominant role of adenosine triphosphate-sensitive K ( + ) current in switching on and off the repetitive firing of action potentials at 8 mM ( G ) was taken over at a higher ( G ) by Ca ( 2 + ) - or Na ( + ) - dependent currents , which were generated by the plasma membrane Ca ( 2 + ) pump , Na ( + ) / K ( + ) pump , Na ( + ) / Ca ( 2 + ) exchanger , and TRPM channel .
	manualset3
160959	11	411635	7	NULL	NULL	0	NULL	repetitive firing 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The predominant role of adenosine triphosphate-sensitive K ( + ) current in switching on and off the repetitive firing of action potentials at 8 mM ( G ) was taken over at a higher ( G ) by Ca ( 2 + ) - or Na ( + ) - dependent currents , which were generated by the plasma membrane Ca ( 2 + ) pump , Na ( + ) / K ( + ) pump , Na ( + ) / Ca ( 2 + ) exchanger , and TRPM channel .
	manualset3
160963	12	411635	7	NULL	NULL	0	NULL	switching on and off 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The predominant role of adenosine triphosphate-sensitive K ( + ) current in switching on and off the repetitive firing of action potentials at 8 mM ( G ) was taken over at a higher ( G ) by Ca ( 2 + ) - or Na ( + ) - dependent currents , which were generated by the plasma membrane Ca ( 2 + ) pump , Na ( + ) / K ( + ) pump , Na ( + ) / Ca ( 2 + ) exchanger , and TRPM channel .
	manualset3
159628	1	411636	7	NULL	NULL	0	NULL	duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The preexisting duration of this painful problem did not influence the response to therapy .
	manualset3
159629	2	411636	7	NULL	NULL	0	NULL	painful problem	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The preexisting duration of this painful problem did not influence the response to therapy .
	manualset3
159630	3	411636	7	NULL	NULL	0	NULL	 response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The preexisting duration of this painful problem did not influence the response to therapy .
	manualset3
159631	4	411636	7	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The preexisting duration of this painful problem did not influence the response to therapy .
	manualset3
159632	1	411637	7	NULL	NULL	0	NULL	pregnancy hormones	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The pregnancy hormones human chorionic gonadotropin and progesterone induce human embryonic stem cell proliferation and differentiation into neuroectodermal rosettes .
	manualset3
159633	2	411637	7	NULL	NULL	0	NULL	human chorionic gonadotropin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The pregnancy hormones human chorionic gonadotropin and progesterone induce human embryonic stem cell proliferation and differentiation into neuroectodermal rosettes .
	manualset3
159634	3	411637	7	NULL	NULL	0	NULL	progesterone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The pregnancy hormones human chorionic gonadotropin and progesterone induce human embryonic stem cell proliferation and differentiation into neuroectodermal rosettes .
	manualset3
159635	4	411637	7	NULL	NULL	0	NULL	human embryonic stem cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The pregnancy hormones human chorionic gonadotropin and progesterone induce human embryonic stem cell proliferation and differentiation into neuroectodermal rosettes .
	manualset3
159636	5	411637	7	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The pregnancy hormones human chorionic gonadotropin and progesterone induce human embryonic stem cell proliferation and differentiation into neuroectodermal rosettes .
	manualset3
159637	6	411637	7	NULL	NULL	NULL	NULL	neuroectodermal rosettes	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The pregnancy hormones human chorionic gonadotropin and progesterone induce human embryonic stem cell proliferation and differentiation into neuroectodermal rosettes .
	manualset3
159638	1	411638	7	NULL	NULL	0	NULL	Clinical significance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical significance of pain at the right iliac fossa ) .
	manualset3
159639	2	411638	7	NULL	NULL	0	NULL	pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical significance of pain at the right iliac fossa ) .
	manualset3
159640	3	411638	7	NULL	NULL	0	NULL	right iliac fossa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical significance of pain at the right iliac fossa ) .
	manualset3
159641	1	411639	7	NULL	NULL	0	NULL	preoperative nursing care plan	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The preoperative nursing care plan is developed to meet the physical needs of the child as well as provide essential information and emotional support to the child and family .
	manualset3
159642	2	411639	7	NULL	NULL	0	NULL	 physical needs	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The preoperative nursing care plan is developed to meet the physical needs of the child as well as provide essential information and emotional support to the child and family .
	manualset3
159643	3	411639	7	NULL	NULL	0	NULL	child 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The preoperative nursing care plan is developed to meet the physical needs of the child as well as provide essential information and emotional support to the child and family .
	manualset3
159644	4	411639	7	NULL	NULL	0	NULL	information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The preoperative nursing care plan is developed to meet the physical needs of the child as well as provide essential information and emotional support to the child and family .
	manualset3
159645	5	411639	7	NULL	NULL	0	NULL	emotional support	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The preoperative nursing care plan is developed to meet the physical needs of the child as well as provide essential information and emotional support to the child and family .
	manualset3
159646	6	411639	7	NULL	NULL	0	NULL	child	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The preoperative nursing care plan is developed to meet the physical needs of the child as well as provide essential information and emotional support to the child and family .
	manualset3
159647	7	411639	7	NULL	NULL	0	NULL	family	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The preoperative nursing care plan is developed to meet the physical needs of the child as well as provide essential information and emotional support to the child and family .
	manualset3
159648	1	411640	7	NULL	NULL	NULL	NULL	presence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The presence in the fluids of 13-18 and 20-32 kD components active towards ciliary neurons is consistent with the release of fibroblast growth factor and ciliary neurotrophic factor respectively .
	manualset3
159649	2	411640	7	NULL	NULL	0	NULL	fluids	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence in the fluids of 13-18 and 20-32 kD components active towards ciliary neurons is consistent with the release of fibroblast growth factor and ciliary neurotrophic factor respectively .
	manualset3
159650	3	411640	7	NULL	NULL	0	NULL	13-18 and 20-32 kD components	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence in the fluids of 13-18 and 20-32 kD components active towards ciliary neurons is consistent with the release of fibroblast growth factor and ciliary neurotrophic factor respectively .
	manualset3
159651	4	411640	7	NULL	NULL	0	NULL	ciliary neurons	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence in the fluids of 13-18 and 20-32 kD components active towards ciliary neurons is consistent with the release of fibroblast growth factor and ciliary neurotrophic factor respectively .
	manualset3
159652	5	411640	7	NULL	NULL	0	NULL	release	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence in the fluids of 13-18 and 20-32 kD components active towards ciliary neurons is consistent with the release of fibroblast growth factor and ciliary neurotrophic factor respectively .
	manualset3
159653	6	411640	7	NULL	NULL	NULL	NULL	fibroblast growth factor	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The presence in the fluids of 13-18 and 20-32 kD components active towards ciliary neurons is consistent with the release of fibroblast growth factor and ciliary neurotrophic factor respectively .
	manualset3
159654	7	411640	7	NULL	NULL	NULL	NULL	ciliary neurotrophic factor 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The presence in the fluids of 13-18 and 20-32 kD components active towards ciliary neurons is consistent with the release of fibroblast growth factor and ciliary neurotrophic factor respectively .
	manualset3
159655	1	411641	7	NULL	NULL	0	NULL	ATP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of ATP , adenylyl imidodiphosphate , CaCl2 or higher concentrations of ATPase conferred stability against thermal denaturation , but did not prevent the irreversibility one denaturation had taken place .
	manualset3
159656	2	411641	7	NULL	NULL	0	NULL	adenylyl imidodiphosphate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of ATP , adenylyl imidodiphosphate , CaCl2 or higher concentrations of ATPase conferred stability against thermal denaturation , but did not prevent the irreversibility one denaturation had taken place .
	manualset3
159657	3	411641	7	NULL	NULL	0	NULL	CaCl2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of ATP , adenylyl imidodiphosphate , CaCl2 or higher concentrations of ATPase conferred stability against thermal denaturation , but did not prevent the irreversibility one denaturation had taken place .
	manualset3
159658	4	411641	7	NULL	NULL	0	NULL	ATPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of ATP , adenylyl imidodiphosphate , CaCl2 or higher concentrations of ATPase conferred stability against thermal denaturation , but did not prevent the irreversibility one denaturation had taken place .
	manualset3
159659	5	411641	7	NULL	NULL	0	NULL	thermal denaturation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of ATP , adenylyl imidodiphosphate , CaCl2 or higher concentrations of ATPase conferred stability against thermal denaturation , but did not prevent the irreversibility one denaturation had taken place .
	manualset3
159660	6	411641	7	NULL	NULL	0	NULL	denaturation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of ATP , adenylyl imidodiphosphate , CaCl2 or higher concentrations of ATPase conferred stability against thermal denaturation , but did not prevent the irreversibility one denaturation had taken place .
	manualset3
159688	7	411641	7	NULL	NULL	0	NULL	presence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of ATP , adenylyl imidodiphosphate , CaCl2 or higher concentrations of ATPase conferred stability against thermal denaturation , but did not prevent the irreversibility one denaturation had taken place .
	manualset3
159661	1	411642	7	NULL	NULL	NULL	NULL	presence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The presence of GFAP and S-100p was not correlated with the degree of differentiation in astrocytomas .
	manualset3
159662	2	411642	7	NULL	NULL	0	NULL	GFAP 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of GFAP and S-100p was not correlated with the degree of differentiation in astrocytomas .
	manualset3
159663	3	411642	7	NULL	NULL	0	NULL	S-100p	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of GFAP and S-100p was not correlated with the degree of differentiation in astrocytomas .
	manualset3
159664	4	411642	7	NULL	NULL	0	NULL	degree of differentiation	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of GFAP and S-100p was not correlated with the degree of differentiation in astrocytomas .
	manualset3
159665	5	411642	7	NULL	NULL	0	NULL	astrocytomas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of GFAP and S-100p was not correlated with the degree of differentiation in astrocytomas .
	manualset3
159666	1	411643	7	NULL	NULL	0	NULL	PVA copolymer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of PVA and poly ( ODA-co-PA ) copolymer on the corresponding particles was shown by FTIR-DRS .
	manualset3
159667	2	411643	7	NULL	NULL	0	NULL	poly ( ODA-co-PA ) copolymer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of PVA and poly ( ODA-co-PA ) copolymer on the corresponding particles was shown by FTIR-DRS .
	manualset3
159668	3	411643	7	NULL	NULL	0	NULL	particles	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of PVA and poly ( ODA-co-PA ) copolymer on the corresponding particles was shown by FTIR-DRS .
	manualset3
159669	4	411643	7	NULL	NULL	0	NULL	FTIR-DRS	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of PVA and poly ( ODA-co-PA ) copolymer on the corresponding particles was shown by FTIR-DRS .
	manualset3
159670	5	411643	7	NULL	NULL	NULL	NULL	presence	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The presence of PVA and poly ( ODA-co-PA ) copolymer on the corresponding particles was shown by FTIR-DRS .
	manualset3
159671	1	411644	7	NULL	NULL	0	NULL	presence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of a binary repeat contributes to the instability of this region of chromosome 17 , yet two CMT1A-REP elements are present in the chimpanzee and all human populations .
	manualset3
159672	2	411644	7	NULL	NULL	0	NULL	binary repeat 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of a binary repeat contributes to the instability of this region of chromosome 17 , yet two CMT1A-REP elements are present in the chimpanzee and all human populations .
	manualset3
159673	3	411644	7	NULL	NULL	NULL	NULL	region	Chromosome												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The presence of a binary repeat contributes to the instability of this region of chromosome 17 , yet two CMT1A-REP elements are present in the chimpanzee and all human populations .
	manualset3
159674	4	411644	7	NULL	NULL	0	NULL	chromosome 17 	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of a binary repeat contributes to the instability of this region of chromosome 17 , yet two CMT1A-REP elements are present in the chimpanzee and all human populations .
	manualset3
159675	5	411644	7	NULL	NULL	0	NULL	CMT1A-REP elements	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of a binary repeat contributes to the instability of this region of chromosome 17 , yet two CMT1A-REP elements are present in the chimpanzee and all human populations .
	manualset3
159676	6	411644	7	NULL	NULL	0	NULL	 chimpanzee	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of a binary repeat contributes to the instability of this region of chromosome 17 , yet two CMT1A-REP elements are present in the chimpanzee and all human populations .
	manualset3
159677	7	411644	7	NULL	NULL	NULL	NULL	human populations	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The presence of a binary repeat contributes to the instability of this region of chromosome 17 , yet two CMT1A-REP elements are present in the chimpanzee and all human populations .
	manualset3
169182	8	411644	7	NULL	NULL	0	NULL	instability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of a binary repeat contributes to the instability of this region of chromosome 17 , yet two CMT1A-REP elements are present in the chimpanzee and all human populations .
	manualset3
159678	1	411645	7	NULL	NULL	0	NULL	 presence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of a bulky residue at this position , such as a tyrosine or phenylalanine , may contribute towards molecular interactions that allow for the enhanced activation with LCA and novel activation with chole .
	manualset3
159679	2	411645	7	NULL	NULL	0	NULL	bulky residue	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of a bulky residue at this position , such as a tyrosine or phenylalanine , may contribute towards molecular interactions that allow for the enhanced activation with LCA and novel activation with chole .
	manualset3
159680	3	411645	7	NULL	NULL	0	NULL	position	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of a bulky residue at this position , such as a tyrosine or phenylalanine , may contribute towards molecular interactions that allow for the enhanced activation with LCA and novel activation with chole .
	manualset3
159681	4	411645	7	NULL	NULL	0	NULL	tyrosine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of a bulky residue at this position , such as a tyrosine or phenylalanine , may contribute towards molecular interactions that allow for the enhanced activation with LCA and novel activation with chole .
	manualset3
159682	5	411645	7	NULL	NULL	0	NULL	phenylalanine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of a bulky residue at this position , such as a tyrosine or phenylalanine , may contribute towards molecular interactions that allow for the enhanced activation with LCA and novel activation with chole .
	manualset3
159683	6	411645	7	NULL	NULL	0	NULL	molecular interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of a bulky residue at this position , such as a tyrosine or phenylalanine , may contribute towards molecular interactions that allow for the enhanced activation with LCA and novel activation with chole .
	manualset3
159684	7	411645	7	NULL	NULL	0	NULL	enhanced activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of a bulky residue at this position , such as a tyrosine or phenylalanine , may contribute towards molecular interactions that allow for the enhanced activation with LCA and novel activation with chole .
	manualset3
159685	8	411645	7	NULL	NULL	0	NULL	LCA	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of a bulky residue at this position , such as a tyrosine or phenylalanine , may contribute towards molecular interactions that allow for the enhanced activation with LCA and novel activation with chole .
	manualset3
159686	9	411645	7	NULL	NULL	0	NULL	novel activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of a bulky residue at this position , such as a tyrosine or phenylalanine , may contribute towards molecular interactions that allow for the enhanced activation with LCA and novel activation with chole .
	manualset3
159687	10	411645	7	NULL	NULL	0	NULL	chole	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of a bulky residue at this position , such as a tyrosine or phenylalanine , may contribute towards molecular interactions that allow for the enhanced activation with LCA and novel activation with chole .
	manualset3
159689	1	411646	7	NULL	NULL	NULL	NULL	presence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The presence of a major gene for uterine capacity ( UC ) , ovulation rate ( OR ) , number of implanted embryos ( IE ) , embryo survival ( ES ) , fetal survival ( FS ) , and prenatal survival ( PS ) was investigated in a population of rabbits divergently selected for UC for 10 generations .
	manualset3
159690	2	411646	7	NULL	NULL	0	NULL	gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of a major gene for uterine capacity ( UC ) , ovulation rate ( OR ) , number of implanted embryos ( IE ) , embryo survival ( ES ) , fetal survival ( FS ) , and prenatal survival ( PS ) was investigated in a population of rabbits divergently selected for UC for 10 generations .
	manualset3
159691	3	411646	7	NULL	NULL	0	NULL	uterine capacity ( UC )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of a major gene for uterine capacity ( UC ) , ovulation rate ( OR ) , number of implanted embryos ( IE ) , embryo survival ( ES ) , fetal survival ( FS ) , and prenatal survival ( PS ) was investigated in a population of rabbits divergently selected for UC for 10 generations .
	manualset3
159692	4	411646	7	NULL	NULL	NULL	NULL	ovulation rate ( OR )	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The presence of a major gene for uterine capacity ( UC ) , ovulation rate ( OR ) , number of implanted embryos ( IE ) , embryo survival ( ES ) , fetal survival ( FS ) , and prenatal survival ( PS ) was investigated in a population of rabbits divergently selected for UC for 10 generations .
	manualset3
159693	5	411646	7	NULL	NULL	0	NULL	embryo survival ( ES )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of a major gene for uterine capacity ( UC ) , ovulation rate ( OR ) , number of implanted embryos ( IE ) , embryo survival ( ES ) , fetal survival ( FS ) , and prenatal survival ( PS ) was investigated in a population of rabbits divergently selected for UC for 10 generations .
	manualset3
159694	6	411646	7	NULL	NULL	0	NULL	fetal survival ( FS )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of a major gene for uterine capacity ( UC ) , ovulation rate ( OR ) , number of implanted embryos ( IE ) , embryo survival ( ES ) , fetal survival ( FS ) , and prenatal survival ( PS ) was investigated in a population of rabbits divergently selected for UC for 10 generations .
	manualset3
159695	7	411646	7	NULL	NULL	0	NULL	prenatal survival ( PS ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of a major gene for uterine capacity ( UC ) , ovulation rate ( OR ) , number of implanted embryos ( IE ) , embryo survival ( ES ) , fetal survival ( FS ) , and prenatal survival ( PS ) was investigated in a population of rabbits divergently selected for UC for 10 generations .
	manualset3
159696	8	411646	7	NULL	NULL	0	NULL	 population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of a major gene for uterine capacity ( UC ) , ovulation rate ( OR ) , number of implanted embryos ( IE ) , embryo survival ( ES ) , fetal survival ( FS ) , and prenatal survival ( PS ) was investigated in a population of rabbits divergently selected for UC for 10 generations .
	manualset3
159697	9	411646	7	NULL	NULL	0	NULL	 rabbits	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of a major gene for uterine capacity ( UC ) , ovulation rate ( OR ) , number of implanted embryos ( IE ) , embryo survival ( ES ) , fetal survival ( FS ) , and prenatal survival ( PS ) was investigated in a population of rabbits divergently selected for UC for 10 generations .
	manualset3
159698	10	411646	7	NULL	NULL	0	NULL	UC 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of a major gene for uterine capacity ( UC ) , ovulation rate ( OR ) , number of implanted embryos ( IE ) , embryo survival ( ES ) , fetal survival ( FS ) , and prenatal survival ( PS ) was investigated in a population of rabbits divergently selected for UC for 10 generations .
	manualset3
159699	11	411646	7	NULL	NULL	NULL	NULL	10 generations	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The presence of a major gene for uterine capacity ( UC ) , ovulation rate ( OR ) , number of implanted embryos ( IE ) , embryo survival ( ES ) , fetal survival ( FS ) , and prenatal survival ( PS ) was investigated in a population of rabbits divergently selected for UC for 10 generations .
	manualset3
160960	12	411646	7	NULL	NULL	NULL	NULL	 number of implanted embryos ( IE )	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The presence of a major gene for uterine capacity ( UC ) , ovulation rate ( OR ) , number of implanted embryos ( IE ) , embryo survival ( ES ) , fetal survival ( FS ) , and prenatal survival ( PS ) was investigated in a population of rabbits divergently selected for UC for 10 generations .
	manualset3
159700	1	411647	7	NULL	NULL	0	NULL	 presence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of alkyl thiol surfactant within the GNF channels changes the dynamics of the AuNP transformations , as surfactant molecules adsorbed on the surface of the AuNPs diminished the stabilization effect of the step-edges , thus allowing nanoparticles to grow until their diameters reach the internal diameter of the host nanofiber .
	manualset3
159701	2	411647	7	NULL	NULL	0	NULL	alkyl thiol surfactant	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of alkyl thiol surfactant within the GNF channels changes the dynamics of the AuNP transformations , as surfactant molecules adsorbed on the surface of the AuNPs diminished the stabilization effect of the step-edges , thus allowing nanoparticles to grow until their diameters reach the internal diameter of the host nanofiber .
	manualset3
159702	3	411647	7	NULL	NULL	0	NULL	GNF channels 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of alkyl thiol surfactant within the GNF channels changes the dynamics of the AuNP transformations , as surfactant molecules adsorbed on the surface of the AuNPs diminished the stabilization effect of the step-edges , thus allowing nanoparticles to grow until their diameters reach the internal diameter of the host nanofiber .
	manualset3
159703	4	411647	7	NULL	NULL	0	NULL	dynamics	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of alkyl thiol surfactant within the GNF channels changes the dynamics of the AuNP transformations , as surfactant molecules adsorbed on the surface of the AuNPs diminished the stabilization effect of the step-edges , thus allowing nanoparticles to grow until their diameters reach the internal diameter of the host nanofiber .
	manualset3
159704	5	411647	7	NULL	NULL	0	NULL	 AuNP transformations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of alkyl thiol surfactant within the GNF channels changes the dynamics of the AuNP transformations , as surfactant molecules adsorbed on the surface of the AuNPs diminished the stabilization effect of the step-edges , thus allowing nanoparticles to grow until their diameters reach the internal diameter of the host nanofiber .
	manualset3
159705	6	411647	7	NULL	NULL	0	NULL	surfactant molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of alkyl thiol surfactant within the GNF channels changes the dynamics of the AuNP transformations , as surfactant molecules adsorbed on the surface of the AuNPs diminished the stabilization effect of the step-edges , thus allowing nanoparticles to grow until their diameters reach the internal diameter of the host nanofiber .
	manualset3
159706	7	411647	7	NULL	NULL	NULL	NULL	surface	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The presence of alkyl thiol surfactant within the GNF channels changes the dynamics of the AuNP transformations , as surfactant molecules adsorbed on the surface of the AuNPs diminished the stabilization effect of the step-edges , thus allowing nanoparticles to grow until their diameters reach the internal diameter of the host nanofiber .
	manualset3
159707	8	411647	7	NULL	NULL	0	NULL	 AuNPs	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of alkyl thiol surfactant within the GNF channels changes the dynamics of the AuNP transformations , as surfactant molecules adsorbed on the surface of the AuNPs diminished the stabilization effect of the step-edges , thus allowing nanoparticles to grow until their diameters reach the internal diameter of the host nanofiber .
	manualset3
159708	9	411647	7	NULL	NULL	0	NULL	stabilization effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of alkyl thiol surfactant within the GNF channels changes the dynamics of the AuNP transformations , as surfactant molecules adsorbed on the surface of the AuNPs diminished the stabilization effect of the step-edges , thus allowing nanoparticles to grow until their diameters reach the internal diameter of the host nanofiber .
	manualset3
159709	10	411647	7	NULL	NULL	0	NULL	step-edges	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of alkyl thiol surfactant within the GNF channels changes the dynamics of the AuNP transformations , as surfactant molecules adsorbed on the surface of the AuNPs diminished the stabilization effect of the step-edges , thus allowing nanoparticles to grow until their diameters reach the internal diameter of the host nanofiber .
	manualset3
159710	11	411647	7	NULL	NULL	0	NULL	nanoparticles	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of alkyl thiol surfactant within the GNF channels changes the dynamics of the AuNP transformations , as surfactant molecules adsorbed on the surface of the AuNPs diminished the stabilization effect of the step-edges , thus allowing nanoparticles to grow until their diameters reach the internal diameter of the host nanofiber .
	manualset3
159711	12	411647	7	NULL	NULL	0	NULL	diameters	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of alkyl thiol surfactant within the GNF channels changes the dynamics of the AuNP transformations , as surfactant molecules adsorbed on the surface of the AuNPs diminished the stabilization effect of the step-edges , thus allowing nanoparticles to grow until their diameters reach the internal diameter of the host nanofiber .
	manualset3
159712	13	411647	7	NULL	NULL	0	NULL	internal diameter 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of alkyl thiol surfactant within the GNF channels changes the dynamics of the AuNP transformations , as surfactant molecules adsorbed on the surface of the AuNPs diminished the stabilization effect of the step-edges , thus allowing nanoparticles to grow until their diameters reach the internal diameter of the host nanofiber .
	manualset3
159713	14	411647	7	NULL	NULL	0	NULL	host nanofiber 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of alkyl thiol surfactant within the GNF channels changes the dynamics of the AuNP transformations , as surfactant molecules adsorbed on the surface of the AuNPs diminished the stabilization effect of the step-edges , thus allowing nanoparticles to grow until their diameters reach the internal diameter of the host nanofiber .
	manualset3
159714	1	411648	7	NULL	NULL	NULL	NULL	presence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The presence of an acute phase response may pre-date the eventual diagnosis of malignant disease by months or even years .
	manualset3
159715	2	411648	7	NULL	NULL	0	NULL	acute phase response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of an acute phase response may pre-date the eventual diagnosis of malignant disease by months or even years .
	manualset3
159716	3	411648	7	NULL	NULL	0	NULL	pre-date 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of an acute phase response may pre-date the eventual diagnosis of malignant disease by months or even years .
	manualset3
159717	4	411648	7	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of an acute phase response may pre-date the eventual diagnosis of malignant disease by months or even years .
	manualset3
159718	5	411648	7	NULL	NULL	0	NULL	malignant disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of an acute phase response may pre-date the eventual diagnosis of malignant disease by months or even years .
	manualset3
159719	6	411648	7	NULL	NULL	0	NULL	 months 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of an acute phase response may pre-date the eventual diagnosis of malignant disease by months or even years .
	manualset3
159720	7	411648	7	NULL	NULL	0	NULL	years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of an acute phase response may pre-date the eventual diagnosis of malignant disease by months or even years .
	manualset3
159721	1	411649	7	NULL	NULL	0	NULL	presence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of antisalivary duct antibody was found in sera from mice with sialadenitis .
	manualset3
159722	2	411649	7	NULL	NULL	NULL	NULL	antisalivary duct antibody	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The presence of antisalivary duct antibody was found in sera from mice with sialadenitis .
	manualset3
159723	3	411649	7	NULL	NULL	0	NULL	sera	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of antisalivary duct antibody was found in sera from mice with sialadenitis .
	manualset3
159724	4	411649	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of antisalivary duct antibody was found in sera from mice with sialadenitis .
	manualset3
159725	5	411649	7	NULL	NULL	0	NULL	sialadenitis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of antisalivary duct antibody was found in sera from mice with sialadenitis .
	manualset3
159726	1	411650	7	NULL	NULL	0	NULL	presence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of barium resulted in a steady-state GABA-induced depolarization of 10.3 + / - 2.0 mV .
	manualset3
159727	2	411650	7	NULL	NULL	0	NULL	barium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of barium resulted in a steady-state GABA-induced depolarization of 10.3 + / - 2.0 mV .
	manualset3
159728	3	411650	7	NULL	NULL	0	NULL	GABA-induced depolarization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of barium resulted in a steady-state GABA-induced depolarization of 10.3 + / - 2.0 mV .
	manualset3
159729	4	411650	7	NULL	NULL	0	NULL	10.3 + / - 2.0 mV	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of barium resulted in a steady-state GABA-induced depolarization of 10.3 + / - 2.0 mV .
	manualset3
159730	1	411651	7	NULL	NULL	0	NULL	presence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of blue-green algae ( BGA ) toxins in surface waters used for drinking water sources and recreation is receiving increasing attention around the world as a public health concern .
	manualset3
159731	2	411651	7	NULL	NULL	0	NULL	blue-green algae ( BGA ) toxins	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of blue-green algae ( BGA ) toxins in surface waters used for drinking water sources and recreation is receiving increasing attention around the world as a public health concern .
	manualset3
159732	3	411651	7	NULL	NULL	0	NULL	surface waters	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of blue-green algae ( BGA ) toxins in surface waters used for drinking water sources and recreation is receiving increasing attention around the world as a public health concern .
	manualset3
159733	4	411651	7	NULL	NULL	0	NULL	drinking water sources	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of blue-green algae ( BGA ) toxins in surface waters used for drinking water sources and recreation is receiving increasing attention around the world as a public health concern .
	manualset3
159734	5	411651	7	NULL	NULL	0	NULL	recreation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of blue-green algae ( BGA ) toxins in surface waters used for drinking water sources and recreation is receiving increasing attention around the world as a public health concern .
	manualset3
159735	6	411651	7	NULL	NULL	0	NULL	attention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of blue-green algae ( BGA ) toxins in surface waters used for drinking water sources and recreation is receiving increasing attention around the world as a public health concern .
	manualset3
159736	7	411651	7	NULL	NULL	0	NULL	world	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of blue-green algae ( BGA ) toxins in surface waters used for drinking water sources and recreation is receiving increasing attention around the world as a public health concern .
	manualset3
159737	8	411651	7	NULL	NULL	0	NULL	public health concern 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of blue-green algae ( BGA ) toxins in surface waters used for drinking water sources and recreation is receiving increasing attention around the world as a public health concern .
	manualset3
159738	1	411652	7	NULL	NULL	0	NULL	 presence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of bromodeoxyuridine in the nuclei of occasional cells that would be counted as neurons on the basis of size and morphology indicates that a process of apparent neurogenesis may underlie the profile of sensory neuron loss after axotomy .
	manualset3
159739	2	411652	7	NULL	NULL	0	NULL	bromodeoxyuridine	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of bromodeoxyuridine in the nuclei of occasional cells that would be counted as neurons on the basis of size and morphology indicates that a process of apparent neurogenesis may underlie the profile of sensory neuron loss after axotomy .
	manualset3
159740	3	411652	7	NULL	NULL	0	NULL	nuclei	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of bromodeoxyuridine in the nuclei of occasional cells that would be counted as neurons on the basis of size and morphology indicates that a process of apparent neurogenesis may underlie the profile of sensory neuron loss after axotomy .
	manualset3
159741	4	411652	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of bromodeoxyuridine in the nuclei of occasional cells that would be counted as neurons on the basis of size and morphology indicates that a process of apparent neurogenesis may underlie the profile of sensory neuron loss after axotomy .
	manualset3
159742	5	411652	7	NULL	NULL	0	NULL	neurons	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of bromodeoxyuridine in the nuclei of occasional cells that would be counted as neurons on the basis of size and morphology indicates that a process of apparent neurogenesis may underlie the profile of sensory neuron loss after axotomy .
	manualset3
159743	6	411652	7	NULL	NULL	0	NULL	size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of bromodeoxyuridine in the nuclei of occasional cells that would be counted as neurons on the basis of size and morphology indicates that a process of apparent neurogenesis may underlie the profile of sensory neuron loss after axotomy .
	manualset3
159744	7	411652	7	NULL	NULL	0	NULL	morphology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of bromodeoxyuridine in the nuclei of occasional cells that would be counted as neurons on the basis of size and morphology indicates that a process of apparent neurogenesis may underlie the profile of sensory neuron loss after axotomy .
	manualset3
159745	8	411652	7	NULL	NULL	0	NULL	process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of bromodeoxyuridine in the nuclei of occasional cells that would be counted as neurons on the basis of size and morphology indicates that a process of apparent neurogenesis may underlie the profile of sensory neuron loss after axotomy .
	manualset3
159746	9	411652	7	NULL	NULL	0	NULL	neurogenesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of bromodeoxyuridine in the nuclei of occasional cells that would be counted as neurons on the basis of size and morphology indicates that a process of apparent neurogenesis may underlie the profile of sensory neuron loss after axotomy .
	manualset3
159747	10	411652	7	NULL	NULL	0	NULL	profile	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of bromodeoxyuridine in the nuclei of occasional cells that would be counted as neurons on the basis of size and morphology indicates that a process of apparent neurogenesis may underlie the profile of sensory neuron loss after axotomy .
	manualset3
159748	11	411652	7	NULL	NULL	0	NULL	sensory neuron loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of bromodeoxyuridine in the nuclei of occasional cells that would be counted as neurons on the basis of size and morphology indicates that a process of apparent neurogenesis may underlie the profile of sensory neuron loss after axotomy .
	manualset3
159749	12	411652	7	NULL	NULL	0	NULL	axotomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of bromodeoxyuridine in the nuclei of occasional cells that would be counted as neurons on the basis of size and morphology indicates that a process of apparent neurogenesis may underlie the profile of sensory neuron loss after axotomy .
	manualset3
159750	1	411653	7	NULL	NULL	NULL	NULL	ANGII	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ANGII showed a significant increase of the wall-to-lumen ratio , perivascular and myocardial fibrosis , and type I collagen mRNA expression , with all these parameters being significantly improved by TCV-116 .
	manualset3
159751	2	411653	7	NULL	NULL	0	NULL	wall-to-lumen ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	ANGII showed a significant increase of the wall-to-lumen ratio , perivascular and myocardial fibrosis , and type I collagen mRNA expression , with all these parameters being significantly improved by TCV-116 .
	manualset3
159752	3	411653	7	NULL	NULL	0	NULL	 perivascular fibrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	ANGII showed a significant increase of the wall-to-lumen ratio , perivascular and myocardial fibrosis , and type I collagen mRNA expression , with all these parameters being significantly improved by TCV-116 .
	manualset3
159753	4	411653	7	NULL	NULL	0	NULL	myocardial fibrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	ANGII showed a significant increase of the wall-to-lumen ratio , perivascular and myocardial fibrosis , and type I collagen mRNA expression , with all these parameters being significantly improved by TCV-116 .
	manualset3
159754	5	411653	7	NULL	NULL	0	NULL	type I collagen mRNA expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	ANGII showed a significant increase of the wall-to-lumen ratio , perivascular and myocardial fibrosis , and type I collagen mRNA expression , with all these parameters being significantly improved by TCV-116 .
	manualset3
159755	6	411653	7	NULL	NULL	0	NULL	parameters	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	ANGII showed a significant increase of the wall-to-lumen ratio , perivascular and myocardial fibrosis , and type I collagen mRNA expression , with all these parameters being significantly improved by TCV-116 .
	manualset3
159756	7	411653	7	NULL	NULL	0	NULL	TCV-116	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	ANGII showed a significant increase of the wall-to-lumen ratio , perivascular and myocardial fibrosis , and type I collagen mRNA expression , with all these parameters being significantly improved by TCV-116 .
	manualset3
169183	8	411653	7	NULL	NULL	0	NULL	significant increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	ANGII showed a significant increase of the wall-to-lumen ratio , perivascular and myocardial fibrosis , and type I collagen mRNA expression , with all these parameters being significantly improved by TCV-116 .
	manualset3
159757	1	411654	7	NULL	NULL	0	NULL	presence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of endosulfan sulfate in the tissues can not be considered as ` detoxification ' which is as toxic as the parent compound .
	manualset3
159758	2	411654	7	NULL	NULL	0	NULL	endosulfan sulfate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of endosulfan sulfate in the tissues can not be considered as ` detoxification ' which is as toxic as the parent compound .
	manualset3
159759	3	411654	7	NULL	NULL	0	NULL	tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of endosulfan sulfate in the tissues can not be considered as ` detoxification ' which is as toxic as the parent compound .
	manualset3
159760	4	411654	7	NULL	NULL	0	NULL	detoxification 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of endosulfan sulfate in the tissues can not be considered as ` detoxification ' which is as toxic as the parent compound .
	manualset3
159761	5	411654	7	NULL	NULL	0	NULL	 parent compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of endosulfan sulfate in the tissues can not be considered as ` detoxification ' which is as toxic as the parent compound .
	manualset3
159762	1	411655	7	NULL	NULL	0	NULL	presence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of extracellular Mn2 + ( 0.5-1 mM ) , which suppresses several Ca2 + - dependent K + currents , also did not affect the slowly inactivating outward current .
	manualset3
159763	2	411655	7	NULL	NULL	0	NULL	extracellular Mn2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of extracellular Mn2 + ( 0.5-1 mM ) , which suppresses several Ca2 + - dependent K + currents , also did not affect the slowly inactivating outward current .
	manualset3
159764	3	411655	7	NULL	NULL	0	NULL	 0.5-1 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of extracellular Mn2 + ( 0.5-1 mM ) , which suppresses several Ca2 + - dependent K + currents , also did not affect the slowly inactivating outward current .
	manualset3
159765	4	411655	7	NULL	NULL	0	NULL	Ca2 + - dependent K + currents	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of extracellular Mn2 + ( 0.5-1 mM ) , which suppresses several Ca2 + - dependent K + currents , also did not affect the slowly inactivating outward current .
	manualset3
159766	5	411655	7	NULL	NULL	0	NULL	outward current 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of extracellular Mn2 + ( 0.5-1 mM ) , which suppresses several Ca2 + - dependent K + currents , also did not affect the slowly inactivating outward current .
	manualset3
159767	1	411656	7	NULL	NULL	NULL	NULL	 presence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The presence of genetic variants may also decrease the sensitivity to pharmacological agents acting through molecular targets or signaling pathways .
	manualset3
159768	2	411656	7	NULL	NULL	NULL	NULL	genetic variants	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The presence of genetic variants may also decrease the sensitivity to pharmacological agents acting through molecular targets or signaling pathways .
	manualset3
159769	3	411656	7	NULL	NULL	NULL	NULL	pharmacological agents 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The presence of genetic variants may also decrease the sensitivity to pharmacological agents acting through molecular targets or signaling pathways .
	manualset3
159770	4	411656	7	NULL	NULL	NULL	NULL	molecular targets	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The presence of genetic variants may also decrease the sensitivity to pharmacological agents acting through molecular targets or signaling pathways .
	manualset3
159771	5	411656	7	NULL	NULL	0	NULL	signaling pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of genetic variants may also decrease the sensitivity to pharmacological agents acting through molecular targets or signaling pathways .
	manualset3
160961	6	411656	7	NULL	NULL	NULL	NULL	sensitivity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The presence of genetic variants may also decrease the sensitivity to pharmacological agents acting through molecular targets or signaling pathways .
	manualset3
159772	1	411657	7	NULL	NULL	0	NULL	presence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of large amounts of PG II in both the seminal vesicle and central zone lends support to the hypothesis of a common mesodermal origin for these two structures .
	manualset3
159773	2	411657	7	NULL	NULL	0	NULL	large amounts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of large amounts of PG II in both the seminal vesicle and central zone lends support to the hypothesis of a common mesodermal origin for these two structures .
	manualset3
159774	3	411657	7	NULL	NULL	0	NULL	PG II 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of large amounts of PG II in both the seminal vesicle and central zone lends support to the hypothesis of a common mesodermal origin for these two structures .
	manualset3
159775	4	411657	7	NULL	NULL	0	NULL	seminal vesicle 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of large amounts of PG II in both the seminal vesicle and central zone lends support to the hypothesis of a common mesodermal origin for these two structures .
	manualset3
159776	5	411657	7	NULL	NULL	0	NULL	central zone	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of large amounts of PG II in both the seminal vesicle and central zone lends support to the hypothesis of a common mesodermal origin for these two structures .
	manualset3
159777	6	411657	7	NULL	NULL	0	NULL	hypothesis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of large amounts of PG II in both the seminal vesicle and central zone lends support to the hypothesis of a common mesodermal origin for these two structures .
	manualset3
159778	7	411657	7	NULL	NULL	0	NULL	mesodermal origin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of large amounts of PG II in both the seminal vesicle and central zone lends support to the hypothesis of a common mesodermal origin for these two structures .
	manualset3
159779	8	411657	7	NULL	NULL	0	NULL	structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of large amounts of PG II in both the seminal vesicle and central zone lends support to the hypothesis of a common mesodermal origin for these two structures .
	manualset3
159780	1	411658	7	NULL	NULL	0	NULL	presence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of leptin in stomach epithelium was recently demonstrated in the rat and humans , and gastric leptin has been linked to the control of meal size , local inflammatory responses , and paracrine and autocrine functions through leptin receptors in the stomach .
	manualset3
159781	2	411658	7	NULL	NULL	0	NULL	leptin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of leptin in stomach epithelium was recently demonstrated in the rat and humans , and gastric leptin has been linked to the control of meal size , local inflammatory responses , and paracrine and autocrine functions through leptin receptors in the stomach .
	manualset3
159782	3	411658	7	NULL	NULL	0	NULL	stomach epithelium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of leptin in stomach epithelium was recently demonstrated in the rat and humans , and gastric leptin has been linked to the control of meal size , local inflammatory responses , and paracrine and autocrine functions through leptin receptors in the stomach .
	manualset3
159783	4	411658	7	NULL	NULL	0	NULL	 rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of leptin in stomach epithelium was recently demonstrated in the rat and humans , and gastric leptin has been linked to the control of meal size , local inflammatory responses , and paracrine and autocrine functions through leptin receptors in the stomach .
	manualset3
159784	5	411658	7	NULL	NULL	0	NULL	humans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of leptin in stomach epithelium was recently demonstrated in the rat and humans , and gastric leptin has been linked to the control of meal size , local inflammatory responses , and paracrine and autocrine functions through leptin receptors in the stomach .
	manualset3
159785	6	411658	7	NULL	NULL	0	NULL	gastric leptin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of leptin in stomach epithelium was recently demonstrated in the rat and humans , and gastric leptin has been linked to the control of meal size , local inflammatory responses , and paracrine and autocrine functions through leptin receptors in the stomach .
	manualset3
159786	7	411658	7	NULL	NULL	0	NULL	 control of meal size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of leptin in stomach epithelium was recently demonstrated in the rat and humans , and gastric leptin has been linked to the control of meal size , local inflammatory responses , and paracrine and autocrine functions through leptin receptors in the stomach .
	manualset3
159787	8	411658	7	NULL	NULL	0	NULL	local inflammatory responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of leptin in stomach epithelium was recently demonstrated in the rat and humans , and gastric leptin has been linked to the control of meal size , local inflammatory responses , and paracrine and autocrine functions through leptin receptors in the stomach .
	manualset3
159788	9	411658	7	NULL	NULL	0	NULL	paracrine functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of leptin in stomach epithelium was recently demonstrated in the rat and humans , and gastric leptin has been linked to the control of meal size , local inflammatory responses , and paracrine and autocrine functions through leptin receptors in the stomach .
	manualset3
159789	10	411658	7	NULL	NULL	0	NULL	autocrine functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of leptin in stomach epithelium was recently demonstrated in the rat and humans , and gastric leptin has been linked to the control of meal size , local inflammatory responses , and paracrine and autocrine functions through leptin receptors in the stomach .
	manualset3
159790	11	411658	7	NULL	NULL	0	NULL	leptin receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of leptin in stomach epithelium was recently demonstrated in the rat and humans , and gastric leptin has been linked to the control of meal size , local inflammatory responses , and paracrine and autocrine functions through leptin receptors in the stomach .
	manualset3
159791	12	411658	7	NULL	NULL	0	NULL	stomach	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of leptin in stomach epithelium was recently demonstrated in the rat and humans , and gastric leptin has been linked to the control of meal size , local inflammatory responses , and paracrine and autocrine functions through leptin receptors in the stomach .
	manualset3
159792	1	411659	7	NULL	NULL	0	NULL	 presence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of maternal antibodies did not interfere significantly with the seroresponse to two doses of IPV-E .
	manualset3
159793	2	411659	7	NULL	NULL	0	NULL	maternal antibodies 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of maternal antibodies did not interfere significantly with the seroresponse to two doses of IPV-E .
	manualset3
159794	3	411659	7	NULL	NULL	0	NULL	seroresponse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of maternal antibodies did not interfere significantly with the seroresponse to two doses of IPV-E .
	manualset3
159795	4	411659	7	NULL	NULL	0	NULL	two doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of maternal antibodies did not interfere significantly with the seroresponse to two doses of IPV-E .
	manualset3
159796	5	411659	7	NULL	NULL	0	NULL	 IPV-E	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of maternal antibodies did not interfere significantly with the seroresponse to two doses of IPV-E .
	manualset3
159797	1	411660	7	NULL	NULL	0	NULL	presence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of metabolic alkalosis , hypokalemia , hypochloremia , and high renin and aldosterone levels were suggestive of Bartter syndrome and a treatment regimen for Bartter syndrome was started .
	manualset3
159798	2	411660	7	NULL	NULL	0	NULL	 metabolic alkalosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of metabolic alkalosis , hypokalemia , hypochloremia , and high renin and aldosterone levels were suggestive of Bartter syndrome and a treatment regimen for Bartter syndrome was started .
	manualset3
159799	3	411660	7	NULL	NULL	0	NULL	hypokalemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of metabolic alkalosis , hypokalemia , hypochloremia , and high renin and aldosterone levels were suggestive of Bartter syndrome and a treatment regimen for Bartter syndrome was started .
	manualset3
159800	4	411660	7	NULL	NULL	0	NULL	hypochloremia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of metabolic alkalosis , hypokalemia , hypochloremia , and high renin and aldosterone levels were suggestive of Bartter syndrome and a treatment regimen for Bartter syndrome was started .
	manualset3
159801	5	411660	7	NULL	NULL	0	NULL	high renin levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of metabolic alkalosis , hypokalemia , hypochloremia , and high renin and aldosterone levels were suggestive of Bartter syndrome and a treatment regimen for Bartter syndrome was started .
	manualset3
159802	6	411660	7	NULL	NULL	0	NULL	aldosterone levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of metabolic alkalosis , hypokalemia , hypochloremia , and high renin and aldosterone levels were suggestive of Bartter syndrome and a treatment regimen for Bartter syndrome was started .
	manualset3
159803	7	411660	7	NULL	NULL	0	NULL	Bartter syndrome 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of metabolic alkalosis , hypokalemia , hypochloremia , and high renin and aldosterone levels were suggestive of Bartter syndrome and a treatment regimen for Bartter syndrome was started .
	manualset3
159804	8	411660	7	NULL	NULL	0	NULL	treatment regimen	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of metabolic alkalosis , hypokalemia , hypochloremia , and high renin and aldosterone levels were suggestive of Bartter syndrome and a treatment regimen for Bartter syndrome was started .
	manualset3
159805	9	411660	7	NULL	NULL	0	NULL	Bartter syndrome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of metabolic alkalosis , hypokalemia , hypochloremia , and high renin and aldosterone levels were suggestive of Bartter syndrome and a treatment regimen for Bartter syndrome was started .
	manualset3
159806	1	411661	7	NULL	NULL	NULL	NULL	AOAA	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	AOAA , NH4 + and KB but not Phs or Gln increase the Ca ( 2 + ) - independent release ( Mg2 + replacing Ca2 + ) of radioactivity by 71 % , 71 % and 108 % respectively .
	manualset3
159807	2	411661	7	NULL	NULL	0	NULL	NH4 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	AOAA , NH4 + and KB but not Phs or Gln increase the Ca ( 2 + ) - independent release ( Mg2 + replacing Ca2 + ) of radioactivity by 71 % , 71 % and 108 % respectively .
	manualset3
159808	3	411661	7	NULL	NULL	NULL	NULL	KB 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	AOAA , NH4 + and KB but not Phs or Gln increase the Ca ( 2 + ) - independent release ( Mg2 + replacing Ca2 + ) of radioactivity by 71 % , 71 % and 108 % respectively .
	manualset3
159809	4	411661	7	NULL	NULL	NULL	NULL	Phs	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	AOAA , NH4 + and KB but not Phs or Gln increase the Ca ( 2 + ) - independent release ( Mg2 + replacing Ca2 + ) of radioactivity by 71 % , 71 % and 108 % respectively .
	manualset3
159810	5	411661	7	NULL	NULL	0	NULL	Gln 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	AOAA , NH4 + and KB but not Phs or Gln increase the Ca ( 2 + ) - independent release ( Mg2 + replacing Ca2 + ) of radioactivity by 71 % , 71 % and 108 % respectively .
	manualset3
159811	6	411661	7	NULL	NULL	0	NULL	Ca ( 2 + ) - independent release of radioactivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	AOAA , NH4 + and KB but not Phs or Gln increase the Ca ( 2 + ) - independent release ( Mg2 + replacing Ca2 + ) of radioactivity by 71 % , 71 % and 108 % respectively .
	manualset3
159812	7	411661	7	NULL	NULL	0	NULL	Mg2 + replacing Ca2 + 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	AOAA , NH4 + and KB but not Phs or Gln increase the Ca ( 2 + ) - independent release ( Mg2 + replacing Ca2 + ) of radioactivity by 71 % , 71 % and 108 % respectively .
	manualset3
159813	8	411661	7	NULL	NULL	NULL	NULL	71 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	AOAA , NH4 + and KB but not Phs or Gln increase the Ca ( 2 + ) - independent release ( Mg2 + replacing Ca2 + ) of radioactivity by 71 % , 71 % and 108 % respectively .
	manualset3
159814	9	411661	7	NULL	NULL	0	NULL	71 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	AOAA , NH4 + and KB but not Phs or Gln increase the Ca ( 2 + ) - independent release ( Mg2 + replacing Ca2 + ) of radioactivity by 71 % , 71 % and 108 % respectively .
	manualset3
159815	10	411661	7	NULL	NULL	0	NULL	108 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	AOAA , NH4 + and KB but not Phs or Gln increase the Ca ( 2 + ) - independent release ( Mg2 + replacing Ca2 + ) of radioactivity by 71 % , 71 % and 108 % respectively .
	manualset3
159816	1	411662	7	NULL	NULL	0	NULL	presence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of multiple membrane-bound intracellular compartments is a major feature of eukaryotic cells .
	manualset3
159817	2	411662	7	NULL	NULL	0	NULL	multiple membrane-bound intracellular compartments	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of multiple membrane-bound intracellular compartments is a major feature of eukaryotic cells .
	manualset3
159818	3	411662	7	NULL	NULL	0	NULL	eukaryotic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of multiple membrane-bound intracellular compartments is a major feature of eukaryotic cells .
	manualset3
169184	4	411662	7	NULL	NULL	0	NULL	major feature	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of multiple membrane-bound intracellular compartments is a major feature of eukaryotic cells .
	manualset3
159819	1	411663	7	NULL	NULL	0	NULL	 presence 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of only one high-molecular fraction O-PS was a characteristic feature of all investigated strains .
	manualset3
159820	2	411663	7	NULL	NULL	0	NULL	 one high-molecular fraction O-PS	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of only one high-molecular fraction O-PS was a characteristic feature of all investigated strains .
	manualset3
159821	3	411663	7	NULL	NULL	0	NULL	strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of only one high-molecular fraction O-PS was a characteristic feature of all investigated strains .
	manualset3
169185	4	411663	7	NULL	NULL	0	NULL	characteristic feature	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of only one high-molecular fraction O-PS was a characteristic feature of all investigated strains .
	manualset3
159822	1	411664	7	NULL	NULL	0	NULL	presence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of oppositely charged surfactants exhibited a pronounced effect on the dye sorption-low concentrations of the surfactant enhanced sorption , whereas high concentrations solubilized the dyes and kept them in solution .
	manualset3
159823	2	411664	7	NULL	NULL	NULL	NULL	oppositely charged surfactants	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The presence of oppositely charged surfactants exhibited a pronounced effect on the dye sorption-low concentrations of the surfactant enhanced sorption , whereas high concentrations solubilized the dyes and kept them in solution .
	manualset3
159824	3	411664	7	NULL	NULL	0	NULL	dye sorption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of oppositely charged surfactants exhibited a pronounced effect on the dye sorption-low concentrations of the surfactant enhanced sorption , whereas high concentrations solubilized the dyes and kept them in solution .
	manualset3
159825	4	411664	7	NULL	NULL	0	NULL	low concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of oppositely charged surfactants exhibited a pronounced effect on the dye sorption-low concentrations of the surfactant enhanced sorption , whereas high concentrations solubilized the dyes and kept them in solution .
	manualset3
159826	5	411664	7	NULL	NULL	0	NULL	surfactant	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of oppositely charged surfactants exhibited a pronounced effect on the dye sorption-low concentrations of the surfactant enhanced sorption , whereas high concentrations solubilized the dyes and kept them in solution .
	manualset3
159827	6	411664	7	NULL	NULL	0	NULL	sorption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of oppositely charged surfactants exhibited a pronounced effect on the dye sorption-low concentrations of the surfactant enhanced sorption , whereas high concentrations solubilized the dyes and kept them in solution .
	manualset3
159828	7	411664	7	NULL	NULL	0	NULL	 high concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of oppositely charged surfactants exhibited a pronounced effect on the dye sorption-low concentrations of the surfactant enhanced sorption , whereas high concentrations solubilized the dyes and kept them in solution .
	manualset3
159829	8	411664	7	NULL	NULL	0	NULL	dyes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of oppositely charged surfactants exhibited a pronounced effect on the dye sorption-low concentrations of the surfactant enhanced sorption , whereas high concentrations solubilized the dyes and kept them in solution .
	manualset3
159830	9	411664	7	NULL	NULL	0	NULL	solution	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of oppositely charged surfactants exhibited a pronounced effect on the dye sorption-low concentrations of the surfactant enhanced sorption , whereas high concentrations solubilized the dyes and kept them in solution .
	manualset3
159831	1	411665	7	NULL	NULL	0	NULL	presence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of shared epitopes suggests the possibility of devising a panel of skin test reagents representative of a large group of basidiomycetes .
	manualset3
159832	2	411665	7	NULL	NULL	0	NULL	shared epitopes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of shared epitopes suggests the possibility of devising a panel of skin test reagents representative of a large group of basidiomycetes .
	manualset3
159833	3	411665	7	NULL	NULL	0	NULL	skin test reagents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of shared epitopes suggests the possibility of devising a panel of skin test reagents representative of a large group of basidiomycetes .
	manualset3
159834	4	411665	7	NULL	NULL	0	NULL	large group	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of shared epitopes suggests the possibility of devising a panel of skin test reagents representative of a large group of basidiomycetes .
	manualset3
159835	5	411665	7	NULL	NULL	0	NULL	basidiomycetes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of shared epitopes suggests the possibility of devising a panel of skin test reagents representative of a large group of basidiomycetes .
	manualset3
169186	6	411665	7	NULL	NULL	0	NULL	panel	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of shared epitopes suggests the possibility of devising a panel of skin test reagents representative of a large group of basidiomycetes .
	manualset3
159836	1	411666	7	NULL	NULL	0	NULL	 presence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of shared epitopes between an Epstein-Barr virus protein , BOLF1 , and the hypervariable region of HLA associated with the pauciarticular form of JCA , recently reported , could provide a key to the pathogenesis of other collagen diseases such as scleroderma .
	manualset3
159837	2	411666	7	NULL	NULL	NULL	NULL	shared epitopes	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The presence of shared epitopes between an Epstein-Barr virus protein , BOLF1 , and the hypervariable region of HLA associated with the pauciarticular form of JCA , recently reported , could provide a key to the pathogenesis of other collagen diseases such as scleroderma .
	manualset3
159838	3	411666	7	NULL	NULL	0	NULL	Epstein-Barr virus protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of shared epitopes between an Epstein-Barr virus protein , BOLF1 , and the hypervariable region of HLA associated with the pauciarticular form of JCA , recently reported , could provide a key to the pathogenesis of other collagen diseases such as scleroderma .
	manualset3
159839	4	411666	7	NULL	NULL	0	NULL	BOLF1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of shared epitopes between an Epstein-Barr virus protein , BOLF1 , and the hypervariable region of HLA associated with the pauciarticular form of JCA , recently reported , could provide a key to the pathogenesis of other collagen diseases such as scleroderma .
	manualset3
159840	5	411666	7	NULL	NULL	0	NULL	hypervariable region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of shared epitopes between an Epstein-Barr virus protein , BOLF1 , and the hypervariable region of HLA associated with the pauciarticular form of JCA , recently reported , could provide a key to the pathogenesis of other collagen diseases such as scleroderma .
	manualset3
159841	6	411666	7	NULL	NULL	0	NULL	HLA	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of shared epitopes between an Epstein-Barr virus protein , BOLF1 , and the hypervariable region of HLA associated with the pauciarticular form of JCA , recently reported , could provide a key to the pathogenesis of other collagen diseases such as scleroderma .
	manualset3
159842	7	411666	7	NULL	NULL	0	NULL	pauciarticular form of JCA	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of shared epitopes between an Epstein-Barr virus protein , BOLF1 , and the hypervariable region of HLA associated with the pauciarticular form of JCA , recently reported , could provide a key to the pathogenesis of other collagen diseases such as scleroderma .
	manualset3
159843	8	411666	7	NULL	NULL	0	NULL	key 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of shared epitopes between an Epstein-Barr virus protein , BOLF1 , and the hypervariable region of HLA associated with the pauciarticular form of JCA , recently reported , could provide a key to the pathogenesis of other collagen diseases such as scleroderma .
	manualset3
159844	9	411666	7	NULL	NULL	0	NULL	pathogenesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of shared epitopes between an Epstein-Barr virus protein , BOLF1 , and the hypervariable region of HLA associated with the pauciarticular form of JCA , recently reported , could provide a key to the pathogenesis of other collagen diseases such as scleroderma .
	manualset3
159845	10	411666	7	NULL	NULL	0	NULL	collagen diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of shared epitopes between an Epstein-Barr virus protein , BOLF1 , and the hypervariable region of HLA associated with the pauciarticular form of JCA , recently reported , could provide a key to the pathogenesis of other collagen diseases such as scleroderma .
	manualset3
159846	11	411666	7	NULL	NULL	0	NULL	 scleroderma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of shared epitopes between an Epstein-Barr virus protein , BOLF1 , and the hypervariable region of HLA associated with the pauciarticular form of JCA , recently reported , could provide a key to the pathogenesis of other collagen diseases such as scleroderma .
	manualset3
159847	1	411667	7	NULL	NULL	0	NULL	 presence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of the anionic form of the acids appeared to be essential for derivatization , being diminished in strong acidic conditions .
	manualset3
159848	2	411667	7	NULL	NULL	0	NULL	anionic form of the acids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of the anionic form of the acids appeared to be essential for derivatization , being diminished in strong acidic conditions .
	manualset3
159849	3	411667	7	NULL	NULL	0	NULL	derivatization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of the anionic form of the acids appeared to be essential for derivatization , being diminished in strong acidic conditions .
	manualset3
159850	4	411667	7	NULL	NULL	0	NULL	strong acidic conditions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of the anionic form of the acids appeared to be essential for derivatization , being diminished in strong acidic conditions .
	manualset3
159851	1	411668	7	NULL	NULL	0	NULL	 presence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of this ciliate community agrees with the carbon and nitrogen compounds removal efficiencies .
	manualset3
159852	2	411668	7	NULL	NULL	0	NULL	ciliate community	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of this ciliate community agrees with the carbon and nitrogen compounds removal efficiencies .
	manualset3
159853	3	411668	7	NULL	NULL	0	NULL	carbon compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of this ciliate community agrees with the carbon and nitrogen compounds removal efficiencies .
	manualset3
159854	4	411668	7	NULL	NULL	0	NULL	nitrogen compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of this ciliate community agrees with the carbon and nitrogen compounds removal efficiencies .
	manualset3
169187	5	411668	7	NULL	NULL	0	NULL	removal efficiencies	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of this ciliate community agrees with the carbon and nitrogen compounds removal efficiencies .
	manualset3
159855	1	411669	7	NULL	NULL	0	NULL	presence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of three cytokines also was investigated .
	manualset3
159856	2	411669	7	NULL	NULL	0	NULL	cytokines	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of three cytokines also was investigated .
	manualset3
159857	1	411670	7	NULL	NULL	NULL	NULL	AORN Ergonomic Tool 7	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	AORN Ergonomic Tool 7 : Pushing , Pulling , and Moving Equipment on Wheels can help perioperative team members assess the risk of pushing and pulling tasks in the perioperative setting .
	manualset3
159858	2	411670	7	NULL	NULL	NULL	NULL	Pushing Equipment	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	AORN Ergonomic Tool 7 : Pushing , Pulling , and Moving Equipment on Wheels can help perioperative team members assess the risk of pushing and pulling tasks in the perioperative setting .
	manualset3
159859	3	411670	7	NULL	NULL	0	NULL	Pulling Equipment	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	AORN Ergonomic Tool 7 : Pushing , Pulling , and Moving Equipment on Wheels can help perioperative team members assess the risk of pushing and pulling tasks in the perioperative setting .
	manualset3
159860	4	411670	7	NULL	NULL	0	NULL	Moving Equipment 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	AORN Ergonomic Tool 7 : Pushing , Pulling , and Moving Equipment on Wheels can help perioperative team members assess the risk of pushing and pulling tasks in the perioperative setting .
	manualset3
159861	5	411670	7	NULL	NULL	0	NULL	Wheels 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	AORN Ergonomic Tool 7 : Pushing , Pulling , and Moving Equipment on Wheels can help perioperative team members assess the risk of pushing and pulling tasks in the perioperative setting .
	manualset3
159862	6	411670	7	NULL	NULL	0	NULL	perioperative team members 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	AORN Ergonomic Tool 7 : Pushing , Pulling , and Moving Equipment on Wheels can help perioperative team members assess the risk of pushing and pulling tasks in the perioperative setting .
	manualset3
159863	7	411670	7	NULL	NULL	0	NULL	risk	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	AORN Ergonomic Tool 7 : Pushing , Pulling , and Moving Equipment on Wheels can help perioperative team members assess the risk of pushing and pulling tasks in the perioperative setting .
	manualset3
159864	8	411670	7	NULL	NULL	0	NULL	pushing task	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	AORN Ergonomic Tool 7 : Pushing , Pulling , and Moving Equipment on Wheels can help perioperative team members assess the risk of pushing and pulling tasks in the perioperative setting .
	manualset3
159865	9	411670	7	NULL	NULL	0	NULL	pulling tasks	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	AORN Ergonomic Tool 7 : Pushing , Pulling , and Moving Equipment on Wheels can help perioperative team members assess the risk of pushing and pulling tasks in the perioperative setting .
	manualset3
169188	10	411670	7	NULL	NULL	0	NULL	perioperative setting 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	AORN Ergonomic Tool 7 : Pushing , Pulling , and Moving Equipment on Wheels can help perioperative team members assess the risk of pushing and pulling tasks in the perioperative setting .
	manualset3
159866	1	411671	7	NULL	NULL	0	NULL	presence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of viruses in blood cells or plasma from asymptomatic donors is the major risk of transmitting an infectious agent through blood transfusion .
	manualset3
159867	2	411671	7	NULL	NULL	0	NULL	viruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of viruses in blood cells or plasma from asymptomatic donors is the major risk of transmitting an infectious agent through blood transfusion .
	manualset3
159868	3	411671	7	NULL	NULL	0	NULL	blood cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of viruses in blood cells or plasma from asymptomatic donors is the major risk of transmitting an infectious agent through blood transfusion .
	manualset3
159869	4	411671	7	NULL	NULL	0	NULL	plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of viruses in blood cells or plasma from asymptomatic donors is the major risk of transmitting an infectious agent through blood transfusion .
	manualset3
159870	5	411671	7	NULL	NULL	0	NULL	asymptomatic donors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of viruses in blood cells or plasma from asymptomatic donors is the major risk of transmitting an infectious agent through blood transfusion .
	manualset3
159871	6	411671	7	NULL	NULL	0	NULL	risk	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of viruses in blood cells or plasma from asymptomatic donors is the major risk of transmitting an infectious agent through blood transfusion .
	manualset3
159872	7	411671	7	NULL	NULL	0	NULL	 infectious agent 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of viruses in blood cells or plasma from asymptomatic donors is the major risk of transmitting an infectious agent through blood transfusion .
	manualset3
159873	8	411671	7	NULL	NULL	0	NULL	blood transfusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of viruses in blood cells or plasma from asymptomatic donors is the major risk of transmitting an infectious agent through blood transfusion .
	manualset3
159874	1	411672	7	NULL	NULL	0	NULL	 present article 	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	The present article reports the effect on survival as well as on the morpho-histochemical changes in the trunk kidney of juvenile turbot Scophthalmus maximus , L. induced by acute action of the anionic surfactant , sodium dodecyl sulphate ( SDS ) .
	manualset3
159875	2	411672	7	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present article reports the effect on survival as well as on the morpho-histochemical changes in the trunk kidney of juvenile turbot Scophthalmus maximus , L. induced by acute action of the anionic surfactant , sodium dodecyl sulphate ( SDS ) .
	manualset3
159876	3	411672	7	NULL	NULL	0	NULL	survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present article reports the effect on survival as well as on the morpho-histochemical changes in the trunk kidney of juvenile turbot Scophthalmus maximus , L. induced by acute action of the anionic surfactant , sodium dodecyl sulphate ( SDS ) .
	manualset3
159877	4	411672	7	NULL	NULL	0	NULL	morpho-histochemical changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present article reports the effect on survival as well as on the morpho-histochemical changes in the trunk kidney of juvenile turbot Scophthalmus maximus , L. induced by acute action of the anionic surfactant , sodium dodecyl sulphate ( SDS ) .
	manualset3
159878	5	411672	7	NULL	NULL	0	NULL	trunk kidney 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The present article reports the effect on survival as well as on the morpho-histochemical changes in the trunk kidney of juvenile turbot Scophthalmus maximus , L. induced by acute action of the anionic surfactant , sodium dodecyl sulphate ( SDS ) .
	manualset3
159879	6	411672	7	NULL	NULL	0	NULL	juvenile turbot Scophthalmus maximus , L	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The present article reports the effect on survival as well as on the morpho-histochemical changes in the trunk kidney of juvenile turbot Scophthalmus maximus , L. induced by acute action of the anionic surfactant , sodium dodecyl sulphate ( SDS ) .
	manualset3
159880	7	411672	7	NULL	NULL	0	NULL	anionic surfactant	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present article reports the effect on survival as well as on the morpho-histochemical changes in the trunk kidney of juvenile turbot Scophthalmus maximus , L. induced by acute action of the anionic surfactant , sodium dodecyl sulphate ( SDS ) .
	manualset3
159881	8	411672	7	NULL	NULL	0	NULL	sodium dodecyl sulphate ( SDS )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present article reports the effect on survival as well as on the morpho-histochemical changes in the trunk kidney of juvenile turbot Scophthalmus maximus , L. induced by acute action of the anionic surfactant , sodium dodecyl sulphate ( SDS ) .
	manualset3
169189	9	411672	7	NULL	NULL	0	NULL	acute action	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present article reports the effect on survival as well as on the morpho-histochemical changes in the trunk kidney of juvenile turbot Scophthalmus maximus , L. induced by acute action of the anionic surfactant , sodium dodecyl sulphate ( SDS ) .
	manualset3
159882	1	411673	7	NULL	NULL	0	NULL	computational study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present computational study describes the structure and properties of a substoichiometric 2D monatomic in the height phase of nickel oxide , c ( 4 x 2 ) - Ni ( 3 ) O ( 4 ) , which has been newly found to epitaxially grow under special deposition conditions on the ( 100 ) face of palladium .
	manualset3
159883	2	411673	7	NULL	NULL	0	NULL	structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present computational study describes the structure and properties of a substoichiometric 2D monatomic in the height phase of nickel oxide , c ( 4 x 2 ) - Ni ( 3 ) O ( 4 ) , which has been newly found to epitaxially grow under special deposition conditions on the ( 100 ) face of palladium .
	manualset3
159884	3	411673	7	NULL	NULL	0	NULL	properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present computational study describes the structure and properties of a substoichiometric 2D monatomic in the height phase of nickel oxide , c ( 4 x 2 ) - Ni ( 3 ) O ( 4 ) , which has been newly found to epitaxially grow under special deposition conditions on the ( 100 ) face of palladium .
	manualset3
159885	4	411673	7	NULL	NULL	0	NULL	substoichiometric 2D monatomic	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present computational study describes the structure and properties of a substoichiometric 2D monatomic in the height phase of nickel oxide , c ( 4 x 2 ) - Ni ( 3 ) O ( 4 ) , which has been newly found to epitaxially grow under special deposition conditions on the ( 100 ) face of palladium .
	manualset3
159886	5	411673	7	NULL	NULL	0	NULL	height phase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present computational study describes the structure and properties of a substoichiometric 2D monatomic in the height phase of nickel oxide , c ( 4 x 2 ) - Ni ( 3 ) O ( 4 ) , which has been newly found to epitaxially grow under special deposition conditions on the ( 100 ) face of palladium .
	manualset3
159887	6	411673	7	NULL	NULL	0	NULL	nickel oxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present computational study describes the structure and properties of a substoichiometric 2D monatomic in the height phase of nickel oxide , c ( 4 x 2 ) - Ni ( 3 ) O ( 4 ) , which has been newly found to epitaxially grow under special deposition conditions on the ( 100 ) face of palladium .
	manualset3
159888	7	411673	7	NULL	NULL	0	NULL	c ( 4 x 2 ) - Ni ( 3 ) O ( 4 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The present computational study describes the structure and properties of a substoichiometric 2D monatomic in the height phase of nickel oxide , c ( 4 x 2 ) - Ni ( 3 ) O ( 4 ) , which has been newly found to epitaxially grow under special deposition conditions on the ( 100 ) face of palladium .
	manualset3
159889	8	411673	7	NULL	NULL	0	NULL	special deposition conditions 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The present computational study describes the structure and properties of a substoichiometric 2D monatomic in the height phase of nickel oxide , c ( 4 x 2 ) - Ni ( 3 ) O ( 4 ) , which has been newly found to epitaxially grow under special deposition conditions on the ( 100 ) face of palladium .
	manualset3
159890	9	411673	7	NULL	NULL	0	NULL	 ( 100 ) face	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The present computational study describes the structure and properties of a substoichiometric 2D monatomic in the height phase of nickel oxide , c ( 4 x 2 ) - Ni ( 3 ) O ( 4 ) , which has been newly found to epitaxially grow under special deposition conditions on the ( 100 ) face of palladium .
	manualset3
159891	10	411673	7	NULL	NULL	0	NULL	palladium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present computational study describes the structure and properties of a substoichiometric 2D monatomic in the height phase of nickel oxide , c ( 4 x 2 ) - Ni ( 3 ) O ( 4 ) , which has been newly found to epitaxially grow under special deposition conditions on the ( 100 ) face of palladium .
	manualset3
159892	1	411674	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data , therefore , suggests that there are significant alterations in sphingomyelin , fatty acids and protein profiles between BPH and CAP tissues .
	manualset3
159893	2	411674	7	NULL	NULL	0	NULL	sphingomyelin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data , therefore , suggests that there are significant alterations in sphingomyelin , fatty acids and protein profiles between BPH and CAP tissues .
	manualset3
159894	3	411674	7	NULL	NULL	0	NULL	fatty acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data , therefore , suggests that there are significant alterations in sphingomyelin , fatty acids and protein profiles between BPH and CAP tissues .
	manualset3
159895	4	411674	7	NULL	NULL	0	NULL	protein profiles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data , therefore , suggests that there are significant alterations in sphingomyelin , fatty acids and protein profiles between BPH and CAP tissues .
	manualset3
159896	5	411674	7	NULL	NULL	0	NULL	BPH tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data , therefore , suggests that there are significant alterations in sphingomyelin , fatty acids and protein profiles between BPH and CAP tissues .
	manualset3
159897	6	411674	7	NULL	NULL	0	NULL	CAP tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data , therefore , suggests that there are significant alterations in sphingomyelin , fatty acids and protein profiles between BPH and CAP tissues .
	manualset3
169190	7	411674	7	NULL	NULL	0	NULL	alterations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data , therefore , suggests that there are significant alterations in sphingomyelin , fatty acids and protein profiles between BPH and CAP tissues .
	manualset3
159898	1	411675	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data shows that ETHA and ETHM in therapeutic doses may have M-cholinolytic properties , ETHA being more potent than ETHM .
	manualset3
159899	2	411675	7	NULL	NULL	0	NULL	ETHA	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data shows that ETHA and ETHM in therapeutic doses may have M-cholinolytic properties , ETHA being more potent than ETHM .
	manualset3
159900	3	411675	7	NULL	NULL	0	NULL	ETHM	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data shows that ETHA and ETHM in therapeutic doses may have M-cholinolytic properties , ETHA being more potent than ETHM .
	manualset3
159901	4	411675	7	NULL	NULL	0	NULL	therapeutic doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data shows that ETHA and ETHM in therapeutic doses may have M-cholinolytic properties , ETHA being more potent than ETHM .
	manualset3
159902	5	411675	7	NULL	NULL	0	NULL	M-cholinolytic properties	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data shows that ETHA and ETHM in therapeutic doses may have M-cholinolytic properties , ETHA being more potent than ETHM .
	manualset3
159903	6	411675	7	NULL	NULL	0	NULL	ETHA	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data shows that ETHA and ETHM in therapeutic doses may have M-cholinolytic properties , ETHA being more potent than ETHM .
	manualset3
159904	7	411675	7	NULL	NULL	0	NULL	ETHM	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data shows that ETHA and ETHM in therapeutic doses may have M-cholinolytic properties , ETHA being more potent than ETHM .
	manualset3
159905	1	411676	7	NULL	NULL	0	NULL	 demonstration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present demonstration of Fos activation , in conjunction with differential expression of MR and stimulation of AVP mRNA , suggests that a neuroanatomical pathway comprising the AMYG , osmosensitive brain regions and magnocellular nuclei becomes activated during DOCA effects on salt appetite .
	manualset3
159906	2	411676	7	NULL	NULL	NULL	NULL	Fos activation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present demonstration of Fos activation , in conjunction with differential expression of MR and stimulation of AVP mRNA , suggests that a neuroanatomical pathway comprising the AMYG , osmosensitive brain regions and magnocellular nuclei becomes activated during DOCA effects on salt appetite .
	manualset3
159907	3	411676	7	NULL	NULL	0	NULL	expression of MR 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present demonstration of Fos activation , in conjunction with differential expression of MR and stimulation of AVP mRNA , suggests that a neuroanatomical pathway comprising the AMYG , osmosensitive brain regions and magnocellular nuclei becomes activated during DOCA effects on salt appetite .
	manualset3
159908	4	411676	7	NULL	NULL	0	NULL	stimulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present demonstration of Fos activation , in conjunction with differential expression of MR and stimulation of AVP mRNA , suggests that a neuroanatomical pathway comprising the AMYG , osmosensitive brain regions and magnocellular nuclei becomes activated during DOCA effects on salt appetite .
	manualset3
159909	5	411676	7	NULL	NULL	0	NULL	AVP mRNA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The present demonstration of Fos activation , in conjunction with differential expression of MR and stimulation of AVP mRNA , suggests that a neuroanatomical pathway comprising the AMYG , osmosensitive brain regions and magnocellular nuclei becomes activated during DOCA effects on salt appetite .
	manualset3
159910	6	411676	7	NULL	NULL	0	NULL	neuroanatomical pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present demonstration of Fos activation , in conjunction with differential expression of MR and stimulation of AVP mRNA , suggests that a neuroanatomical pathway comprising the AMYG , osmosensitive brain regions and magnocellular nuclei becomes activated during DOCA effects on salt appetite .
	manualset3
159911	7	411676	7	NULL	NULL	0	NULL	AMYG 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The present demonstration of Fos activation , in conjunction with differential expression of MR and stimulation of AVP mRNA , suggests that a neuroanatomical pathway comprising the AMYG , osmosensitive brain regions and magnocellular nuclei becomes activated during DOCA effects on salt appetite .
	manualset3
159912	8	411676	7	NULL	NULL	0	NULL	osmosensitive brain regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The present demonstration of Fos activation , in conjunction with differential expression of MR and stimulation of AVP mRNA , suggests that a neuroanatomical pathway comprising the AMYG , osmosensitive brain regions and magnocellular nuclei becomes activated during DOCA effects on salt appetite .
	manualset3
159913	9	411676	7	NULL	NULL	0	NULL	magnocellular nuclei	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The present demonstration of Fos activation , in conjunction with differential expression of MR and stimulation of AVP mRNA , suggests that a neuroanatomical pathway comprising the AMYG , osmosensitive brain regions and magnocellular nuclei becomes activated during DOCA effects on salt appetite .
	manualset3
159914	10	411676	7	NULL	NULL	0	NULL	DOCA effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present demonstration of Fos activation , in conjunction with differential expression of MR and stimulation of AVP mRNA , suggests that a neuroanatomical pathway comprising the AMYG , osmosensitive brain regions and magnocellular nuclei becomes activated during DOCA effects on salt appetite .
	manualset3
159915	11	411676	7	NULL	NULL	0	NULL	salt appetite	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present demonstration of Fos activation , in conjunction with differential expression of MR and stimulation of AVP mRNA , suggests that a neuroanatomical pathway comprising the AMYG , osmosensitive brain regions and magnocellular nuclei becomes activated during DOCA effects on salt appetite .
	manualset3
159916	1	411677	7	NULL	NULL	0	NULL	synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present efficient synthesis of ( 5 ' -13 C ) ribonucleosides and 2 ' - deoxy ( 5 ' -13 C ) ribonucleosides is characterized by the synthesis of the D - ( 5-13C ) ribose derivative as an intermediate via the Wittig reaction of 4-aldehydo-D-erythrose dialkyl acetals with Ph3P13CH3I-BuLi to introduce the 13C label at the 5-position of a pentose .
	manualset3
159917	2	411677	7	NULL	NULL	0	NULL	( 5 ' -13 C ) ribonucleosides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present efficient synthesis of ( 5 ' -13 C ) ribonucleosides and 2 ' - deoxy ( 5 ' -13 C ) ribonucleosides is characterized by the synthesis of the D - ( 5-13C ) ribose derivative as an intermediate via the Wittig reaction of 4-aldehydo-D-erythrose dialkyl acetals with Ph3P13CH3I-BuLi to introduce the 13C label at the 5-position of a pentose .
	manualset3
159918	3	411677	7	NULL	NULL	0	NULL	2 ' - deoxy ( 5 ' -13 C ) ribonucleosides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present efficient synthesis of ( 5 ' -13 C ) ribonucleosides and 2 ' - deoxy ( 5 ' -13 C ) ribonucleosides is characterized by the synthesis of the D - ( 5-13C ) ribose derivative as an intermediate via the Wittig reaction of 4-aldehydo-D-erythrose dialkyl acetals with Ph3P13CH3I-BuLi to introduce the 13C label at the 5-position of a pentose .
	manualset3
159919	4	411677	7	NULL	NULL	0	NULL	synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present efficient synthesis of ( 5 ' -13 C ) ribonucleosides and 2 ' - deoxy ( 5 ' -13 C ) ribonucleosides is characterized by the synthesis of the D - ( 5-13C ) ribose derivative as an intermediate via the Wittig reaction of 4-aldehydo-D-erythrose dialkyl acetals with Ph3P13CH3I-BuLi to introduce the 13C label at the 5-position of a pentose .
	manualset3
159920	5	411677	7	NULL	NULL	0	NULL	D - ( 5-13C ) ribose derivative	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present efficient synthesis of ( 5 ' -13 C ) ribonucleosides and 2 ' - deoxy ( 5 ' -13 C ) ribonucleosides is characterized by the synthesis of the D - ( 5-13C ) ribose derivative as an intermediate via the Wittig reaction of 4-aldehydo-D-erythrose dialkyl acetals with Ph3P13CH3I-BuLi to introduce the 13C label at the 5-position of a pentose .
	manualset3
159921	6	411677	7	NULL	NULL	NULL	NULL	Wittig reaction	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present efficient synthesis of ( 5 ' -13 C ) ribonucleosides and 2 ' - deoxy ( 5 ' -13 C ) ribonucleosides is characterized by the synthesis of the D - ( 5-13C ) ribose derivative as an intermediate via the Wittig reaction of 4-aldehydo-D-erythrose dialkyl acetals with Ph3P13CH3I-BuLi to introduce the 13C label at the 5-position of a pentose .
	manualset3
159922	7	411677	7	NULL	NULL	0	NULL	 4-aldehydo-D-erythrose dialkyl acetals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present efficient synthesis of ( 5 ' -13 C ) ribonucleosides and 2 ' - deoxy ( 5 ' -13 C ) ribonucleosides is characterized by the synthesis of the D - ( 5-13C ) ribose derivative as an intermediate via the Wittig reaction of 4-aldehydo-D-erythrose dialkyl acetals with Ph3P13CH3I-BuLi to introduce the 13C label at the 5-position of a pentose .
	manualset3
159923	8	411677	7	NULL	NULL	NULL	NULL	Ph3P13CH3I-BuLi	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present efficient synthesis of ( 5 ' -13 C ) ribonucleosides and 2 ' - deoxy ( 5 ' -13 C ) ribonucleosides is characterized by the synthesis of the D - ( 5-13C ) ribose derivative as an intermediate via the Wittig reaction of 4-aldehydo-D-erythrose dialkyl acetals with Ph3P13CH3I-BuLi to introduce the 13C label at the 5-position of a pentose .
	manualset3
159924	9	411677	7	NULL	NULL	0	NULL	13C label 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present efficient synthesis of ( 5 ' -13 C ) ribonucleosides and 2 ' - deoxy ( 5 ' -13 C ) ribonucleosides is characterized by the synthesis of the D - ( 5-13C ) ribose derivative as an intermediate via the Wittig reaction of 4-aldehydo-D-erythrose dialkyl acetals with Ph3P13CH3I-BuLi to introduce the 13C label at the 5-position of a pentose .
	manualset3
159925	10	411677	7	NULL	NULL	0	NULL	 5-position 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The present efficient synthesis of ( 5 ' -13 C ) ribonucleosides and 2 ' - deoxy ( 5 ' -13 C ) ribonucleosides is characterized by the synthesis of the D - ( 5-13C ) ribose derivative as an intermediate via the Wittig reaction of 4-aldehydo-D-erythrose dialkyl acetals with Ph3P13CH3I-BuLi to introduce the 13C label at the 5-position of a pentose .
	manualset3
159926	11	411677	7	NULL	NULL	0	NULL	pentose	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present efficient synthesis of ( 5 ' -13 C ) ribonucleosides and 2 ' - deoxy ( 5 ' -13 C ) ribonucleosides is characterized by the synthesis of the D - ( 5-13C ) ribose derivative as an intermediate via the Wittig reaction of 4-aldehydo-D-erythrose dialkyl acetals with Ph3P13CH3I-BuLi to introduce the 13C label at the 5-position of a pentose .
	manualset3
159927	1	411678	7	NULL	NULL	0	NULL	experiment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present experiment addressed whether increases in corticospinal excitability following sensory stimulation with muscle tendon vibration are accompanied by reorganization of the forearm musculature representation within the primary motor cortex .
	manualset3
159928	2	411678	7	NULL	NULL	0	NULL	corticospinal excitability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present experiment addressed whether increases in corticospinal excitability following sensory stimulation with muscle tendon vibration are accompanied by reorganization of the forearm musculature representation within the primary motor cortex .
	manualset3
159929	3	411678	7	NULL	NULL	0	NULL	sensory stimulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present experiment addressed whether increases in corticospinal excitability following sensory stimulation with muscle tendon vibration are accompanied by reorganization of the forearm musculature representation within the primary motor cortex .
	manualset3
159930	4	411678	7	NULL	NULL	0	NULL	muscle tendon vibration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present experiment addressed whether increases in corticospinal excitability following sensory stimulation with muscle tendon vibration are accompanied by reorganization of the forearm musculature representation within the primary motor cortex .
	manualset3
159931	5	411678	7	NULL	NULL	0	NULL	reorganization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present experiment addressed whether increases in corticospinal excitability following sensory stimulation with muscle tendon vibration are accompanied by reorganization of the forearm musculature representation within the primary motor cortex .
	manualset3
159932	6	411678	7	NULL	NULL	0	NULL	forearm musculature representation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present experiment addressed whether increases in corticospinal excitability following sensory stimulation with muscle tendon vibration are accompanied by reorganization of the forearm musculature representation within the primary motor cortex .
	manualset3
159933	7	411678	7	NULL	NULL	0	NULL	primary motor cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The present experiment addressed whether increases in corticospinal excitability following sensory stimulation with muscle tendon vibration are accompanied by reorganization of the forearm musculature representation within the primary motor cortex .
	manualset3
159934	1	411679	7	NULL	NULL	0	NULL	findings	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present findings demonstrate that the antimutagenic potential of C. cassia could be attributed to its modulatory effect on the xenobiotic bioactivation and detoxification processes .
	manualset3
159935	2	411679	7	NULL	NULL	0	NULL	antimutagenic potential	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present findings demonstrate that the antimutagenic potential of C. cassia could be attributed to its modulatory effect on the xenobiotic bioactivation and detoxification processes .
	manualset3
159936	3	411679	7	NULL	NULL	0	NULL	C. cassia	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The present findings demonstrate that the antimutagenic potential of C. cassia could be attributed to its modulatory effect on the xenobiotic bioactivation and detoxification processes .
	manualset3
159937	4	411679	7	NULL	NULL	0	NULL	 xenobiotic bioactivation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present findings demonstrate that the antimutagenic potential of C. cassia could be attributed to its modulatory effect on the xenobiotic bioactivation and detoxification processes .
	manualset3
159938	5	411679	7	NULL	NULL	NULL	NULL	detoxification processes	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present findings demonstrate that the antimutagenic potential of C. cassia could be attributed to its modulatory effect on the xenobiotic bioactivation and detoxification processes .
	manualset3
169191	6	411679	7	NULL	NULL	0	NULL	modulatory effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present findings demonstrate that the antimutagenic potential of C. cassia could be attributed to its modulatory effect on the xenobiotic bioactivation and detoxification processes .
	manualset3
159939	1	411680	7	NULL	NULL	0	NULL	investigation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present investigation focuses on the role of the IL-2 receptor in the deficient IF gamma production in neonatal T cells .
	manualset3
159940	2	411680	7	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present investigation focuses on the role of the IL-2 receptor in the deficient IF gamma production in neonatal T cells .
	manualset3
159941	3	411680	7	NULL	NULL	0	NULL	IL-2 receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present investigation focuses on the role of the IL-2 receptor in the deficient IF gamma production in neonatal T cells .
	manualset3
159942	4	411680	7	NULL	NULL	0	NULL	IF gamma production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present investigation focuses on the role of the IL-2 receptor in the deficient IF gamma production in neonatal T cells .
	manualset3
159943	5	411680	7	NULL	NULL	0	NULL	neonatal T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The present investigation focuses on the role of the IL-2 receptor in the deficient IF gamma production in neonatal T cells .
	manualset3
159944	1	411681	7	NULL	NULL	0	NULL	APC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	APC stimulates the GEF activity of Asef and Asef2 , and thereby regulates cell adhesion and migration .
	manualset3
159945	2	411681	7	NULL	NULL	0	NULL	GEF activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	APC stimulates the GEF activity of Asef and Asef2 , and thereby regulates cell adhesion and migration .
	manualset3
159946	3	411681	7	NULL	NULL	0	NULL	Asef	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	APC stimulates the GEF activity of Asef and Asef2 , and thereby regulates cell adhesion and migration .
	manualset3
159947	4	411681	7	NULL	NULL	0	NULL	Asef2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	APC stimulates the GEF activity of Asef and Asef2 , and thereby regulates cell adhesion and migration .
	manualset3
159948	5	411681	7	NULL	NULL	0	NULL	cell adhesion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	APC stimulates the GEF activity of Asef and Asef2 , and thereby regulates cell adhesion and migration .
	manualset3
159949	6	411681	7	NULL	NULL	0	NULL	migration	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	APC stimulates the GEF activity of Asef and Asef2 , and thereby regulates cell adhesion and migration .
	manualset3
159950	1	411682	7	NULL	NULL	0	NULL	 investigation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present investigation was undertaken to investigate the endogenous status of free radical scavengers during cutaneous wound healing in immunocompromised rats .
	manualset3
159951	2	411682	7	NULL	NULL	0	NULL	endogenous status	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present investigation was undertaken to investigate the endogenous status of free radical scavengers during cutaneous wound healing in immunocompromised rats .
	manualset3
159952	3	411682	7	NULL	NULL	0	NULL	free radical scavengers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present investigation was undertaken to investigate the endogenous status of free radical scavengers during cutaneous wound healing in immunocompromised rats .
	manualset3
159953	4	411682	7	NULL	NULL	0	NULL	cutaneous wound healing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present investigation was undertaken to investigate the endogenous status of free radical scavengers during cutaneous wound healing in immunocompromised rats .
	manualset3
159954	5	411682	7	NULL	NULL	0	NULL	immunocompromised rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The present investigation was undertaken to investigate the endogenous status of free radical scavengers during cutaneous wound healing in immunocompromised rats .
	manualset3
159955	1	411683	7	NULL	NULL	0	NULL	microscope 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The present microscope is coupled to two independently tunable lasers and has two principal configurations : holographic imaging combined with galvo-steered uncaging and holographic uncaging combined with conventional scanning imaging .
	manualset3
159956	2	411683	7	NULL	NULL	NULL	NULL	tunable lasers 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present microscope is coupled to two independently tunable lasers and has two principal configurations : holographic imaging combined with galvo-steered uncaging and holographic uncaging combined with conventional scanning imaging .
	manualset3
159957	3	411683	7	NULL	NULL	0	NULL	principal configurations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present microscope is coupled to two independently tunable lasers and has two principal configurations : holographic imaging combined with galvo-steered uncaging and holographic uncaging combined with conventional scanning imaging .
	manualset3
159958	4	411683	7	NULL	NULL	0	NULL	holographic imaging 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present microscope is coupled to two independently tunable lasers and has two principal configurations : holographic imaging combined with galvo-steered uncaging and holographic uncaging combined with conventional scanning imaging .
	manualset3
159959	5	411683	7	NULL	NULL	0	NULL	galvo-steered uncaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present microscope is coupled to two independently tunable lasers and has two principal configurations : holographic imaging combined with galvo-steered uncaging and holographic uncaging combined with conventional scanning imaging .
	manualset3
159960	6	411683	7	NULL	NULL	0	NULL	holographic uncaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present microscope is coupled to two independently tunable lasers and has two principal configurations : holographic imaging combined with galvo-steered uncaging and holographic uncaging combined with conventional scanning imaging .
	manualset3
159961	7	411683	7	NULL	NULL	0	NULL	conventional scanning imaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present microscope is coupled to two independently tunable lasers and has two principal configurations : holographic imaging combined with galvo-steered uncaging and holographic uncaging combined with conventional scanning imaging .
	manualset3
159962	1	411684	7	NULL	NULL	0	NULL	paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper is confined to a description and discussion of the legal framework of Israel 's expert bioethics regime .
	manualset3
159963	2	411684	7	NULL	NULL	0	NULL	description	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper is confined to a description and discussion of the legal framework of Israel 's expert bioethics regime .
	manualset3
159964	3	411684	7	NULL	NULL	0	NULL	discussion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper is confined to a description and discussion of the legal framework of Israel 's expert bioethics regime .
	manualset3
159965	4	411684	7	NULL	NULL	0	NULL	legal framework 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper is confined to a description and discussion of the legal framework of Israel 's expert bioethics regime .
	manualset3
159966	5	411684	7	NULL	NULL	0	NULL	Israel 's expert bioethics regime	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper is confined to a description and discussion of the legal framework of Israel 's expert bioethics regime .
	manualset3
159967	1	411685	7	NULL	NULL	0	NULL	paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159968	2	411685	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159969	3	411685	7	NULL	NULL	0	NULL	EEDQ	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159970	4	411685	7	NULL	NULL	0	NULL	NAD ( H ) - binding domain 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159971	5	411685	7	NULL	NULL	0	NULL	TH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159972	6	411685	7	NULL	NULL	0	NULL	site	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159973	7	411685	7	NULL	NULL	0	NULL	DCCD 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159974	8	411685	7	NULL	NULL	0	NULL	TH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159975	9	411685	7	NULL	NULL	0	NULL	85 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159976	10	411685	7	NULL	NULL	0	NULL	EEDQ	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159977	11	411685	7	NULL	NULL	0	NULL	( 14C ) DCCD	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159978	12	411685	7	NULL	NULL	0	NULL	70 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159979	13	411685	7	NULL	NULL	0	NULL	maximum	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159980	14	411685	7	NULL	NULL	0	NULL	time period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159981	15	411685	7	NULL	NULL	0	NULL	unmodified TH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159982	16	411685	7	NULL	NULL	0	NULL	( 14C ) DCCD	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159983	17	411685	7	NULL	NULL	0	NULL	1 mol DCCD/TH dimer	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159984	18	411685	7	NULL	NULL	0	NULL	DCCD	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159985	19	411685	7	NULL	NULL	0	NULL	TH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159986	20	411685	7	NULL	NULL	0	NULL	NAD-agarose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159987	21	411685	7	NULL	NULL	0	NULL	EEDQ-modified TH 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159988	22	411685	7	NULL	NULL	0	NULL	partial affinity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159989	23	411685	7	NULL	NULL	0	NULL	NAD-agarose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159990	24	411685	7	NULL	NULL	0	NULL	5 ' - AMP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159991	25	411685	7	NULL	NULL	0	NULL	TH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159992	26	411685	7	NULL	NULL	0	NULL	modification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159993	27	411685	7	NULL	NULL	0	NULL	DCCD	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159994	28	411685	7	NULL	NULL	0	NULL	 protective effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159995	29	411685	7	NULL	NULL	0	NULL	EEDQ	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159996	30	411685	7	NULL	NULL	0	NULL	NMNH	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159997	31	411685	7	NULL	NULL	0	NULL	TH substrate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159998	32	411685	7	NULL	NULL	0	NULL	NADH site	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
159999	33	411685	7	NULL	NULL	0	NULL	TH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
160000	34	411685	7	NULL	NULL	0	NULL	DCCD	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
160001	35	411685	7	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
160002	36	411685	7	NULL	NULL	0	NULL	attack	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
160003	37	411685	7	NULL	NULL	0	NULL	EEDQ	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present paper presents data suggesting that EEDQ also binds at or near the NAD ( H ) - binding domain of TH , but at a site not identical to that of DCCD : TH modified with and inhibited approximately 85 % by EEDQ could be further labeled with ( 14C ) DCCD to the extent of 70 % of the maximum in the same time period that unmodified TH was modified by ( 14C ) DCCD to near saturation ( 1 mol DCCD/TH dimer ) ; DCCD-modified TH did not bind to NAD-agarose , while EEDQ-modified TH showed partial affinity for NAD-agarose ; 5 ' - AMP completely protected TH against modification by DCCD , but showed only a weak protective effect against EEDQ ; by contrast , NMNH , which is a TH substrate and binds to the NADH site , did not protect TH against DCCD , but completely protected the enzyme against attack by EEDQ .
	manualset3
160004	1	411686	7	NULL	NULL	0	NULL	pilot study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present pilot study investigated the pattern of neuropsychological functioning associated with the presence of delusions in mild-to-moderate dementia .
	manualset3
160005	2	411686	7	NULL	NULL	0	NULL	pattern	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present pilot study investigated the pattern of neuropsychological functioning associated with the presence of delusions in mild-to-moderate dementia .
	manualset3
160006	3	411686	7	NULL	NULL	0	NULL	neuropsychological functioning	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present pilot study investigated the pattern of neuropsychological functioning associated with the presence of delusions in mild-to-moderate dementia .
	manualset3
160007	4	411686	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present pilot study investigated the pattern of neuropsychological functioning associated with the presence of delusions in mild-to-moderate dementia .
	manualset3
160008	5	411686	7	NULL	NULL	0	NULL	delusions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present pilot study investigated the pattern of neuropsychological functioning associated with the presence of delusions in mild-to-moderate dementia .
	manualset3
160009	6	411686	7	NULL	NULL	0	NULL	mild-to-moderate dementia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present pilot study investigated the pattern of neuropsychological functioning associated with the presence of delusions in mild-to-moderate dementia .
	manualset3
160010	1	411687	7	NULL	NULL	0	NULL	reagent system	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present reagent system , PIFA/HPA , was also applied to the oxidation of other non-phenolic benzyltetrahydroisoquinolines and the high yield conversion to morphinandienones was accomplished .
	manualset3
160011	2	411687	7	NULL	NULL	0	NULL	 PIFA/HPA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present reagent system , PIFA/HPA , was also applied to the oxidation of other non-phenolic benzyltetrahydroisoquinolines and the high yield conversion to morphinandienones was accomplished .
	manualset3
160012	3	411687	7	NULL	NULL	0	NULL	oxidation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present reagent system , PIFA/HPA , was also applied to the oxidation of other non-phenolic benzyltetrahydroisoquinolines and the high yield conversion to morphinandienones was accomplished .
	manualset3
160013	4	411687	7	NULL	NULL	0	NULL	non-phenolic benzyltetrahydroisoquinolines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present reagent system , PIFA/HPA , was also applied to the oxidation of other non-phenolic benzyltetrahydroisoquinolines and the high yield conversion to morphinandienones was accomplished .
	manualset3
160014	5	411687	7	NULL	NULL	0	NULL	high yield	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present reagent system , PIFA/HPA , was also applied to the oxidation of other non-phenolic benzyltetrahydroisoquinolines and the high yield conversion to morphinandienones was accomplished .
	manualset3
160015	6	411687	7	NULL	NULL	0	NULL	conversion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present reagent system , PIFA/HPA , was also applied to the oxidation of other non-phenolic benzyltetrahydroisoquinolines and the high yield conversion to morphinandienones was accomplished .
	manualset3
160016	7	411687	7	NULL	NULL	0	NULL	morphinandienones	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present reagent system , PIFA/HPA , was also applied to the oxidation of other non-phenolic benzyltetrahydroisoquinolines and the high yield conversion to morphinandienones was accomplished .
	manualset3
160017	1	411688	7	NULL	NULL	0	NULL	report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The present report describes the sequence of activation and deactivation of multiple unit activities ( MUA ) in the brain stem reticular formation and pyramidal tract , in relation to the clinical seizure and electroencephalographic and electromyographic tonic-clonic discharges induced by pentylenetetrazol ( PTZ ) , in cats immobilized by high spinal transection ( ` encphale isol ' ) .
	manualset3
160018	2	411688	7	NULL	NULL	NULL	NULL	sequence of activation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present report describes the sequence of activation and deactivation of multiple unit activities ( MUA ) in the brain stem reticular formation and pyramidal tract , in relation to the clinical seizure and electroencephalographic and electromyographic tonic-clonic discharges induced by pentylenetetrazol ( PTZ ) , in cats immobilized by high spinal transection ( ` encphale isol ' ) .
	manualset3
160019	3	411688	7	NULL	NULL	NULL	NULL	deactivation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present report describes the sequence of activation and deactivation of multiple unit activities ( MUA ) in the brain stem reticular formation and pyramidal tract , in relation to the clinical seizure and electroencephalographic and electromyographic tonic-clonic discharges induced by pentylenetetrazol ( PTZ ) , in cats immobilized by high spinal transection ( ` encphale isol ' ) .
	manualset3
160020	4	411688	7	NULL	NULL	NULL	NULL	multiple unit activities ( MUA )	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present report describes the sequence of activation and deactivation of multiple unit activities ( MUA ) in the brain stem reticular formation and pyramidal tract , in relation to the clinical seizure and electroencephalographic and electromyographic tonic-clonic discharges induced by pentylenetetrazol ( PTZ ) , in cats immobilized by high spinal transection ( ` encphale isol ' ) .
	manualset3
160021	5	411688	7	NULL	NULL	0	NULL	brain stem reticular formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present report describes the sequence of activation and deactivation of multiple unit activities ( MUA ) in the brain stem reticular formation and pyramidal tract , in relation to the clinical seizure and electroencephalographic and electromyographic tonic-clonic discharges induced by pentylenetetrazol ( PTZ ) , in cats immobilized by high spinal transection ( ` encphale isol ' ) .
	manualset3
160022	6	411688	7	NULL	NULL	0	NULL	pyramidal tract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The present report describes the sequence of activation and deactivation of multiple unit activities ( MUA ) in the brain stem reticular formation and pyramidal tract , in relation to the clinical seizure and electroencephalographic and electromyographic tonic-clonic discharges induced by pentylenetetrazol ( PTZ ) , in cats immobilized by high spinal transection ( ` encphale isol ' ) .
	manualset3
160023	7	411688	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The present report describes the sequence of activation and deactivation of multiple unit activities ( MUA ) in the brain stem reticular formation and pyramidal tract , in relation to the clinical seizure and electroencephalographic and electromyographic tonic-clonic discharges induced by pentylenetetrazol ( PTZ ) , in cats immobilized by high spinal transection ( ` encphale isol ' ) .
	manualset3
160024	8	411688	7	NULL	NULL	0	NULL	clinical seizure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present report describes the sequence of activation and deactivation of multiple unit activities ( MUA ) in the brain stem reticular formation and pyramidal tract , in relation to the clinical seizure and electroencephalographic and electromyographic tonic-clonic discharges induced by pentylenetetrazol ( PTZ ) , in cats immobilized by high spinal transection ( ` encphale isol ' ) .
	manualset3
160025	9	411688	7	NULL	NULL	0	NULL	 electroencephalographic tonic-clonic discharges	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The present report describes the sequence of activation and deactivation of multiple unit activities ( MUA ) in the brain stem reticular formation and pyramidal tract , in relation to the clinical seizure and electroencephalographic and electromyographic tonic-clonic discharges induced by pentylenetetrazol ( PTZ ) , in cats immobilized by high spinal transection ( ` encphale isol ' ) .
	manualset3
160026	10	411688	7	NULL	NULL	0	NULL	electromyographic tonic-clonic discharges	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The present report describes the sequence of activation and deactivation of multiple unit activities ( MUA ) in the brain stem reticular formation and pyramidal tract , in relation to the clinical seizure and electroencephalographic and electromyographic tonic-clonic discharges induced by pentylenetetrazol ( PTZ ) , in cats immobilized by high spinal transection ( ` encphale isol ' ) .
	manualset3
160027	11	411688	7	NULL	NULL	0	NULL	 pentylenetetrazol ( PTZ )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present report describes the sequence of activation and deactivation of multiple unit activities ( MUA ) in the brain stem reticular formation and pyramidal tract , in relation to the clinical seizure and electroencephalographic and electromyographic tonic-clonic discharges induced by pentylenetetrazol ( PTZ ) , in cats immobilized by high spinal transection ( ` encphale isol ' ) .
	manualset3
160028	12	411688	7	NULL	NULL	0	NULL	cats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The present report describes the sequence of activation and deactivation of multiple unit activities ( MUA ) in the brain stem reticular formation and pyramidal tract , in relation to the clinical seizure and electroencephalographic and electromyographic tonic-clonic discharges induced by pentylenetetrazol ( PTZ ) , in cats immobilized by high spinal transection ( ` encphale isol ' ) .
	manualset3
160029	13	411688	7	NULL	NULL	0	NULL	high spinal transection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The present report describes the sequence of activation and deactivation of multiple unit activities ( MUA ) in the brain stem reticular formation and pyramidal tract , in relation to the clinical seizure and electroencephalographic and electromyographic tonic-clonic discharges induced by pentylenetetrazol ( PTZ ) , in cats immobilized by high spinal transection ( ` encphale isol ' ) .
	manualset3
160030	14	411688	7	NULL	NULL	0	NULL	encphale isol 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The present report describes the sequence of activation and deactivation of multiple unit activities ( MUA ) in the brain stem reticular formation and pyramidal tract , in relation to the clinical seizure and electroencephalographic and electromyographic tonic-clonic discharges induced by pentylenetetrazol ( PTZ ) , in cats immobilized by high spinal transection ( ` encphale isol ' ) .
	manualset3
160031	1	411689	7	NULL	NULL	0	NULL	APL patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	APL patients expressed with survivin mRNA had DIC and serious infection ( one patient died ) .
	manualset3
160032	2	411689	7	NULL	NULL	0	NULL	survivin mRNA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	APL patients expressed with survivin mRNA had DIC and serious infection ( one patient died ) .
	manualset3
160033	3	411689	7	NULL	NULL	0	NULL	DIC	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	APL patients expressed with survivin mRNA had DIC and serious infection ( one patient died ) .
	manualset3
160034	4	411689	7	NULL	NULL	0	NULL	serious infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	APL patients expressed with survivin mRNA had DIC and serious infection ( one patient died ) .
	manualset3
160035	5	411689	7	NULL	NULL	0	NULL	one patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	APL patients expressed with survivin mRNA had DIC and serious infection ( one patient died ) .
	manualset3
160036	1	411690	7	NULL	NULL	0	NULL	results	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results demonstrate for the first time that down-regulation of MHC expression on individual micrometastatic cells correlates to the differential pattern of metastasis obtained by comparing breast and gastrointestinal carcinomas .
	manualset3
160037	2	411690	7	NULL	NULL	0	NULL	first time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results demonstrate for the first time that down-regulation of MHC expression on individual micrometastatic cells correlates to the differential pattern of metastasis obtained by comparing breast and gastrointestinal carcinomas .
	manualset3
160038	3	411690	7	NULL	NULL	NULL	NULL	down-regulation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present results demonstrate for the first time that down-regulation of MHC expression on individual micrometastatic cells correlates to the differential pattern of metastasis obtained by comparing breast and gastrointestinal carcinomas .
	manualset3
160039	4	411690	7	NULL	NULL	0	NULL	MHC expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results demonstrate for the first time that down-regulation of MHC expression on individual micrometastatic cells correlates to the differential pattern of metastasis obtained by comparing breast and gastrointestinal carcinomas .
	manualset3
160040	5	411690	7	NULL	NULL	0	NULL	micrometastatic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results demonstrate for the first time that down-regulation of MHC expression on individual micrometastatic cells correlates to the differential pattern of metastasis obtained by comparing breast and gastrointestinal carcinomas .
	manualset3
160041	6	411690	7	NULL	NULL	0	NULL	metastasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results demonstrate for the first time that down-regulation of MHC expression on individual micrometastatic cells correlates to the differential pattern of metastasis obtained by comparing breast and gastrointestinal carcinomas .
	manualset3
160042	7	411690	7	NULL	NULL	0	NULL	breast carcinoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results demonstrate for the first time that down-regulation of MHC expression on individual micrometastatic cells correlates to the differential pattern of metastasis obtained by comparing breast and gastrointestinal carcinomas .
	manualset3
160043	8	411690	7	NULL	NULL	0	NULL	gastrointestinal carcinomas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results demonstrate for the first time that down-regulation of MHC expression on individual micrometastatic cells correlates to the differential pattern of metastasis obtained by comparing breast and gastrointestinal carcinomas .
	manualset3
160044	1	411691	7	NULL	NULL	0	NULL	results	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results demonstrate that a relationship exists between the degree of nerve injury-induced galanin expression and the degree of behavioural hypersensitivity , and show that galanin may play a role in nociceptive processing in the spinal cord , with interrelated inhibitory and excitatory effects .
	manualset3
160045	2	411691	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results demonstrate that a relationship exists between the degree of nerve injury-induced galanin expression and the degree of behavioural hypersensitivity , and show that galanin may play a role in nociceptive processing in the spinal cord , with interrelated inhibitory and excitatory effects .
	manualset3
160046	3	411691	7	NULL	NULL	NULL	NULL	degree of nerve injury-induced galanin expression 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present results demonstrate that a relationship exists between the degree of nerve injury-induced galanin expression and the degree of behavioural hypersensitivity , and show that galanin may play a role in nociceptive processing in the spinal cord , with interrelated inhibitory and excitatory effects .
	manualset3
160047	4	411691	7	NULL	NULL	0	NULL	 degree of behavioural hypersensitivity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results demonstrate that a relationship exists between the degree of nerve injury-induced galanin expression and the degree of behavioural hypersensitivity , and show that galanin may play a role in nociceptive processing in the spinal cord , with interrelated inhibitory and excitatory effects .
	manualset3
160048	5	411691	7	NULL	NULL	0	NULL	galanin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results demonstrate that a relationship exists between the degree of nerve injury-induced galanin expression and the degree of behavioural hypersensitivity , and show that galanin may play a role in nociceptive processing in the spinal cord , with interrelated inhibitory and excitatory effects .
	manualset3
160049	6	411691	7	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results demonstrate that a relationship exists between the degree of nerve injury-induced galanin expression and the degree of behavioural hypersensitivity , and show that galanin may play a role in nociceptive processing in the spinal cord , with interrelated inhibitory and excitatory effects .
	manualset3
160050	7	411691	7	NULL	NULL	0	NULL	nociceptive processing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results demonstrate that a relationship exists between the degree of nerve injury-induced galanin expression and the degree of behavioural hypersensitivity , and show that galanin may play a role in nociceptive processing in the spinal cord , with interrelated inhibitory and excitatory effects .
	manualset3
160051	8	411691	7	NULL	NULL	0	NULL	spinal cord	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results demonstrate that a relationship exists between the degree of nerve injury-induced galanin expression and the degree of behavioural hypersensitivity , and show that galanin may play a role in nociceptive processing in the spinal cord , with interrelated inhibitory and excitatory effects .
	manualset3
160052	9	411691	7	NULL	NULL	0	NULL	 interrelated inhibitory effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results demonstrate that a relationship exists between the degree of nerve injury-induced galanin expression and the degree of behavioural hypersensitivity , and show that galanin may play a role in nociceptive processing in the spinal cord , with interrelated inhibitory and excitatory effects .
	manualset3
160053	10	411691	7	NULL	NULL	0	NULL	interrelated excitatory effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results demonstrate that a relationship exists between the degree of nerve injury-induced galanin expression and the degree of behavioural hypersensitivity , and show that galanin may play a role in nociceptive processing in the spinal cord , with interrelated inhibitory and excitatory effects .
	manualset3
160054	1	411692	7	NULL	NULL	0	NULL	results 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results improve those of previous studies using fast atom bombardment and electrospray ionization tanden mass spectrometry , in which it was reported that it was possible to differentiate the identity and position of the sn-2 acyl substituent only by the presence of one ion , with variable abundance .
	manualset3
160055	2	411692	7	NULL	NULL	0	NULL	previous studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results improve those of previous studies using fast atom bombardment and electrospray ionization tanden mass spectrometry , in which it was reported that it was possible to differentiate the identity and position of the sn-2 acyl substituent only by the presence of one ion , with variable abundance .
	manualset3
160056	3	411692	7	NULL	NULL	0	NULL	 fast atom bombardment and electrospray ionization tanden mass spectrometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results improve those of previous studies using fast atom bombardment and electrospray ionization tanden mass spectrometry , in which it was reported that it was possible to differentiate the identity and position of the sn-2 acyl substituent only by the presence of one ion , with variable abundance .
	manualset3
160057	4	411692	7	NULL	NULL	0	NULL	identity	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results improve those of previous studies using fast atom bombardment and electrospray ionization tanden mass spectrometry , in which it was reported that it was possible to differentiate the identity and position of the sn-2 acyl substituent only by the presence of one ion , with variable abundance .
	manualset3
160058	5	411692	7	NULL	NULL	0	NULL	position	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results improve those of previous studies using fast atom bombardment and electrospray ionization tanden mass spectrometry , in which it was reported that it was possible to differentiate the identity and position of the sn-2 acyl substituent only by the presence of one ion , with variable abundance .
	manualset3
160059	6	411692	7	NULL	NULL	0	NULL	sn-2 acyl substituent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results improve those of previous studies using fast atom bombardment and electrospray ionization tanden mass spectrometry , in which it was reported that it was possible to differentiate the identity and position of the sn-2 acyl substituent only by the presence of one ion , with variable abundance .
	manualset3
160060	7	411692	7	NULL	NULL	0	NULL	presence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results improve those of previous studies using fast atom bombardment and electrospray ionization tanden mass spectrometry , in which it was reported that it was possible to differentiate the identity and position of the sn-2 acyl substituent only by the presence of one ion , with variable abundance .
	manualset3
160061	8	411692	7	NULL	NULL	0	NULL	one ion	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results improve those of previous studies using fast atom bombardment and electrospray ionization tanden mass spectrometry , in which it was reported that it was possible to differentiate the identity and position of the sn-2 acyl substituent only by the presence of one ion , with variable abundance .
	manualset3
160062	9	411692	7	NULL	NULL	0	NULL	variable abundance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results improve those of previous studies using fast atom bombardment and electrospray ionization tanden mass spectrometry , in which it was reported that it was possible to differentiate the identity and position of the sn-2 acyl substituent only by the presence of one ion , with variable abundance .
	manualset3
160063	1	411693	7	NULL	NULL	0	NULL	results	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results show that road-race motorcycling imposes a high load on the riders , who should possess adequate fitness to maintain high-speed rides and minimize the effects of fatigue during competition .
	manualset3
160064	2	411693	7	NULL	NULL	0	NULL	road-race motorcycling	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results show that road-race motorcycling imposes a high load on the riders , who should possess adequate fitness to maintain high-speed rides and minimize the effects of fatigue during competition .
	manualset3
160065	3	411693	7	NULL	NULL	0	NULL	high load	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results show that road-race motorcycling imposes a high load on the riders , who should possess adequate fitness to maintain high-speed rides and minimize the effects of fatigue during competition .
	manualset3
160066	4	411693	7	NULL	NULL	0	NULL	riders	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results show that road-race motorcycling imposes a high load on the riders , who should possess adequate fitness to maintain high-speed rides and minimize the effects of fatigue during competition .
	manualset3
160067	5	411693	7	NULL	NULL	NULL	NULL	fitness	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present results show that road-race motorcycling imposes a high load on the riders , who should possess adequate fitness to maintain high-speed rides and minimize the effects of fatigue during competition .
	manualset3
160068	6	411693	7	NULL	NULL	0	NULL	high-speed rides	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results show that road-race motorcycling imposes a high load on the riders , who should possess adequate fitness to maintain high-speed rides and minimize the effects of fatigue during competition .
	manualset3
160069	7	411693	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results show that road-race motorcycling imposes a high load on the riders , who should possess adequate fitness to maintain high-speed rides and minimize the effects of fatigue during competition .
	manualset3
160070	8	411693	7	NULL	NULL	NULL	NULL	fatigue 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present results show that road-race motorcycling imposes a high load on the riders , who should possess adequate fitness to maintain high-speed rides and minimize the effects of fatigue during competition .
	manualset3
160071	9	411693	7	NULL	NULL	0	NULL	competition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results show that road-race motorcycling imposes a high load on the riders , who should possess adequate fitness to maintain high-speed rides and minimize the effects of fatigue during competition .
	manualset3
160072	1	411694	7	NULL	NULL	0	NULL	results	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results show that young and old optic axons course together throughout the depth of the nerve fiber layer .
	manualset3
160073	2	411694	7	NULL	NULL	0	NULL	young optic axons	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results show that young and old optic axons course together throughout the depth of the nerve fiber layer .
	manualset3
160074	3	411694	7	NULL	NULL	0	NULL	old optic axons 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results show that young and old optic axons course together throughout the depth of the nerve fiber layer .
	manualset3
160075	4	411694	7	NULL	NULL	NULL	NULL	depth	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present results show that young and old optic axons course together throughout the depth of the nerve fiber layer .
	manualset3
160076	5	411694	7	NULL	NULL	0	NULL	nerve fiber layer	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The present results show that young and old optic axons course together throughout the depth of the nerve fiber layer .
	manualset3
160077	1	411695	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present studies suggest that in the rat the L-arginine/NO-system not only plays an important role in the regulation of vaginal smooth muscle tone , but also affects blood flow , and may have sensory functions .
	manualset3
160078	2	411695	7	NULL	NULL	0	NULL	 rat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The present studies suggest that in the rat the L-arginine/NO-system not only plays an important role in the regulation of vaginal smooth muscle tone , but also affects blood flow , and may have sensory functions .
	manualset3
160079	3	411695	7	NULL	NULL	NULL	NULL	L-arginine/NO-system	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present studies suggest that in the rat the L-arginine/NO-system not only plays an important role in the regulation of vaginal smooth muscle tone , but also affects blood flow , and may have sensory functions .
	manualset3
160080	4	411695	7	NULL	NULL	0	NULL	 role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present studies suggest that in the rat the L-arginine/NO-system not only plays an important role in the regulation of vaginal smooth muscle tone , but also affects blood flow , and may have sensory functions .
	manualset3
160081	5	411695	7	NULL	NULL	0	NULL	 regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present studies suggest that in the rat the L-arginine/NO-system not only plays an important role in the regulation of vaginal smooth muscle tone , but also affects blood flow , and may have sensory functions .
	manualset3
160082	6	411695	7	NULL	NULL	0	NULL	 vaginal smooth muscle tone	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The present studies suggest that in the rat the L-arginine/NO-system not only plays an important role in the regulation of vaginal smooth muscle tone , but also affects blood flow , and may have sensory functions .
	manualset3
160083	7	411695	7	NULL	NULL	0	NULL	blood flow	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present studies suggest that in the rat the L-arginine/NO-system not only plays an important role in the regulation of vaginal smooth muscle tone , but also affects blood flow , and may have sensory functions .
	manualset3
160084	8	411695	7	NULL	NULL	0	NULL	sensory functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present studies suggest that in the rat the L-arginine/NO-system not only plays an important role in the regulation of vaginal smooth muscle tone , but also affects blood flow , and may have sensory functions .
	manualset3
160085	1	411696	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study analyzed the antioxidative properties of natural compounds from the root of the plant Glycyrrhiza glabra ( licorice ) toward LDL oxidation .
	manualset3
160086	2	411696	7	NULL	NULL	NULL	NULL	antioxidative properties	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present study analyzed the antioxidative properties of natural compounds from the root of the plant Glycyrrhiza glabra ( licorice ) toward LDL oxidation .
	manualset3
160087	3	411696	7	NULL	NULL	0	NULL	 natural compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study analyzed the antioxidative properties of natural compounds from the root of the plant Glycyrrhiza glabra ( licorice ) toward LDL oxidation .
	manualset3
160088	4	411696	7	NULL	NULL	0	NULL	root	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study analyzed the antioxidative properties of natural compounds from the root of the plant Glycyrrhiza glabra ( licorice ) toward LDL oxidation .
	manualset3
160089	5	411696	7	NULL	NULL	0	NULL	plant Glycyrrhiza glabra ( licorice )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study analyzed the antioxidative properties of natural compounds from the root of the plant Glycyrrhiza glabra ( licorice ) toward LDL oxidation .
	manualset3
160090	6	411696	7	NULL	NULL	0	NULL	LDL oxidation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study analyzed the antioxidative properties of natural compounds from the root of the plant Glycyrrhiza glabra ( licorice ) toward LDL oxidation .
	manualset3
160091	1	411697	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study assessed the effect of the inducible isoform , HO-1 .
	manualset3
160092	2	411697	7	NULL	NULL	0	NULL	 effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study assessed the effect of the inducible isoform , HO-1 .
	manualset3
160093	3	411697	7	NULL	NULL	0	NULL	 inducible isoform	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study assessed the effect of the inducible isoform , HO-1 .
	manualset3
160094	4	411697	7	NULL	NULL	0	NULL	HO-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study assessed the effect of the inducible isoform , HO-1 .
	manualset3
160095	1	411698	7	NULL	NULL	0	NULL	APN plan 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	APN plan improves outcome for pregnant patient with congenital heart disease .
	manualset3
160096	2	411698	7	NULL	NULL	0	NULL	 outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	APN plan improves outcome for pregnant patient with congenital heart disease .
	manualset3
160097	3	411698	7	NULL	NULL	0	NULL	pregnant patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	APN plan improves outcome for pregnant patient with congenital heart disease .
	manualset3
160098	4	411698	7	NULL	NULL	0	NULL	congenital heart disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	APN plan improves outcome for pregnant patient with congenital heart disease .
	manualset3
160099	1	411699	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study demonstrated that fascia lata attached anterolateral thigh flaps were useful for reconstructing intractable cranial fistulae complicated by infection .
	manualset3
160100	2	411699	7	NULL	NULL	0	NULL	 fascia lata	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study demonstrated that fascia lata attached anterolateral thigh flaps were useful for reconstructing intractable cranial fistulae complicated by infection .
	manualset3
160101	3	411699	7	NULL	NULL	0	NULL	anterolateral thigh flaps	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study demonstrated that fascia lata attached anterolateral thigh flaps were useful for reconstructing intractable cranial fistulae complicated by infection .
	manualset3
160102	4	411699	7	NULL	NULL	0	NULL	intractable cranial fistulae	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study demonstrated that fascia lata attached anterolateral thigh flaps were useful for reconstructing intractable cranial fistulae complicated by infection .
	manualset3
160103	5	411699	7	NULL	NULL	0	NULL	infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study demonstrated that fascia lata attached anterolateral thigh flaps were useful for reconstructing intractable cranial fistulae complicated by infection .
	manualset3
160104	1	411700	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study demonstrates that a consistent percentage ( over 30 % ) of freshly isolated human Langerhans cells express the CD23 moiety .
	manualset3
160105	2	411700	7	NULL	NULL	0	NULL	consistent percentage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study demonstrates that a consistent percentage ( over 30 % ) of freshly isolated human Langerhans cells express the CD23 moiety .
	manualset3
160106	3	411700	7	NULL	NULL	NULL	NULL	30 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present study demonstrates that a consistent percentage ( over 30 % ) of freshly isolated human Langerhans cells express the CD23 moiety .
	manualset3
160107	4	411700	7	NULL	NULL	0	NULL	human Langerhans cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study demonstrates that a consistent percentage ( over 30 % ) of freshly isolated human Langerhans cells express the CD23 moiety .
	manualset3
160108	5	411700	7	NULL	NULL	0	NULL	CD23 moiety	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study demonstrates that a consistent percentage ( over 30 % ) of freshly isolated human Langerhans cells express the CD23 moiety .
	manualset3
160109	1	411701	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study demonstrates that the last parameters clearly express histological effects induced by UVB irradiation .
	manualset3
160110	2	411701	7	NULL	NULL	0	NULL	 parameters 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study demonstrates that the last parameters clearly express histological effects induced by UVB irradiation .
	manualset3
160111	3	411701	7	NULL	NULL	0	NULL	histological effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study demonstrates that the last parameters clearly express histological effects induced by UVB irradiation .
	manualset3
160112	4	411701	7	NULL	NULL	0	NULL	 UVB irradiation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study demonstrates that the last parameters clearly express histological effects induced by UVB irradiation .
	manualset3
160113	1	411702	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study demonstrates that the neuronal groups in the medial part of lamina VI and the central part of lamina VII of lower cervical segments project to the vermis of the caudal lobules of the anterior lobe and the rostral lobules of the posterior lobe .
	manualset3
160114	2	411702	7	NULL	NULL	0	NULL	neuronal groups 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study demonstrates that the neuronal groups in the medial part of lamina VI and the central part of lamina VII of lower cervical segments project to the vermis of the caudal lobules of the anterior lobe and the rostral lobules of the posterior lobe .
	manualset3
160115	3	411702	7	NULL	NULL	0	NULL	medial part of lamina VI	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study demonstrates that the neuronal groups in the medial part of lamina VI and the central part of lamina VII of lower cervical segments project to the vermis of the caudal lobules of the anterior lobe and the rostral lobules of the posterior lobe .
	manualset3
160116	4	411702	7	NULL	NULL	0	NULL	central part of lamina VII of lower cervical segments	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study demonstrates that the neuronal groups in the medial part of lamina VI and the central part of lamina VII of lower cervical segments project to the vermis of the caudal lobules of the anterior lobe and the rostral lobules of the posterior lobe .
	manualset3
160117	5	411702	7	NULL	NULL	0	NULL	vermis of the caudal lobules of the anterior lobe 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study demonstrates that the neuronal groups in the medial part of lamina VI and the central part of lamina VII of lower cervical segments project to the vermis of the caudal lobules of the anterior lobe and the rostral lobules of the posterior lobe .
	manualset3
160118	6	411702	7	NULL	NULL	0	NULL	rostral lobules of the posterior lobe	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study demonstrates that the neuronal groups in the medial part of lamina VI and the central part of lamina VII of lower cervical segments project to the vermis of the caudal lobules of the anterior lobe and the rostral lobules of the posterior lobe .
	manualset3
160119	1	411703	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study evaluated the effects of intermittent hypoxia ( IH ) and sleep restriction ( SR ) upon motor and cognitive function in rats .
	manualset3
160120	2	411703	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study evaluated the effects of intermittent hypoxia ( IH ) and sleep restriction ( SR ) upon motor and cognitive function in rats .
	manualset3
160121	3	411703	7	NULL	NULL	0	NULL	intermittent hypoxia ( IH )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study evaluated the effects of intermittent hypoxia ( IH ) and sleep restriction ( SR ) upon motor and cognitive function in rats .
	manualset3
160122	4	411703	7	NULL	NULL	0	NULL	sleep restriction ( SR )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study evaluated the effects of intermittent hypoxia ( IH ) and sleep restriction ( SR ) upon motor and cognitive function in rats .
	manualset3
160123	5	411703	7	NULL	NULL	0	NULL	motor function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study evaluated the effects of intermittent hypoxia ( IH ) and sleep restriction ( SR ) upon motor and cognitive function in rats .
	manualset3
160124	6	411703	7	NULL	NULL	0	NULL	cognitive function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study evaluated the effects of intermittent hypoxia ( IH ) and sleep restriction ( SR ) upon motor and cognitive function in rats .
	manualset3
160125	7	411703	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study evaluated the effects of intermittent hypoxia ( IH ) and sleep restriction ( SR ) upon motor and cognitive function in rats .
	manualset3
160126	1	411704	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study examined the prevalence of dementia , anxiety syndromes , depression , psychotic symptoms , sleep disturbance and the use of psychotropic drugs in a population of 330 nonagenarians .
	manualset3
160127	2	411704	7	NULL	NULL	0	NULL	dementia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study examined the prevalence of dementia , anxiety syndromes , depression , psychotic symptoms , sleep disturbance and the use of psychotropic drugs in a population of 330 nonagenarians .
	manualset3
160128	3	411704	7	NULL	NULL	0	NULL	anxiety syndromes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study examined the prevalence of dementia , anxiety syndromes , depression , psychotic symptoms , sleep disturbance and the use of psychotropic drugs in a population of 330 nonagenarians .
	manualset3
160129	4	411704	7	NULL	NULL	0	NULL	depression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study examined the prevalence of dementia , anxiety syndromes , depression , psychotic symptoms , sleep disturbance and the use of psychotropic drugs in a population of 330 nonagenarians .
	manualset3
160130	5	411704	7	NULL	NULL	0	NULL	psychotic symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study examined the prevalence of dementia , anxiety syndromes , depression , psychotic symptoms , sleep disturbance and the use of psychotropic drugs in a population of 330 nonagenarians .
	manualset3
160131	6	411704	7	NULL	NULL	0	NULL	sleep disturbance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study examined the prevalence of dementia , anxiety syndromes , depression , psychotic symptoms , sleep disturbance and the use of psychotropic drugs in a population of 330 nonagenarians .
	manualset3
160132	7	411704	7	NULL	NULL	0	NULL	psychotropic drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study examined the prevalence of dementia , anxiety syndromes , depression , psychotic symptoms , sleep disturbance and the use of psychotropic drugs in a population of 330 nonagenarians .
	manualset3
160133	8	411704	7	NULL	NULL	0	NULL	population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study examined the prevalence of dementia , anxiety syndromes , depression , psychotic symptoms , sleep disturbance and the use of psychotropic drugs in a population of 330 nonagenarians .
	manualset3
160134	9	411704	7	NULL	NULL	0	NULL	 330 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study examined the prevalence of dementia , anxiety syndromes , depression , psychotic symptoms , sleep disturbance and the use of psychotropic drugs in a population of 330 nonagenarians .
	manualset3
160135	10	411704	7	NULL	NULL	0	NULL	nonagenarians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study examined the prevalence of dementia , anxiety syndromes , depression , psychotic symptoms , sleep disturbance and the use of psychotropic drugs in a population of 330 nonagenarians .
	manualset3
160136	1	411705	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study explored the possibility that estrogen enhances the inhibitory effect of an angiotensin II type-1 ( AT1 ) receptor blocker ( ARB ) , olmesartan , on atherosclerosis , focusing on oxidative stress using apolipoprotein E knockout mice ( ApoEKO ) .
	manualset3
160137	2	411705	7	NULL	NULL	0	NULL	possibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study explored the possibility that estrogen enhances the inhibitory effect of an angiotensin II type-1 ( AT1 ) receptor blocker ( ARB ) , olmesartan , on atherosclerosis , focusing on oxidative stress using apolipoprotein E knockout mice ( ApoEKO ) .
	manualset3
160138	3	411705	7	NULL	NULL	0	NULL	estrogen	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study explored the possibility that estrogen enhances the inhibitory effect of an angiotensin II type-1 ( AT1 ) receptor blocker ( ARB ) , olmesartan , on atherosclerosis , focusing on oxidative stress using apolipoprotein E knockout mice ( ApoEKO ) .
	manualset3
160139	4	411705	7	NULL	NULL	0	NULL	inhibitory effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study explored the possibility that estrogen enhances the inhibitory effect of an angiotensin II type-1 ( AT1 ) receptor blocker ( ARB ) , olmesartan , on atherosclerosis , focusing on oxidative stress using apolipoprotein E knockout mice ( ApoEKO ) .
	manualset3
160140	5	411705	7	NULL	NULL	NULL	NULL	angiotensin II type-1 ( AT1 ) receptor blocker ( ARB )	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present study explored the possibility that estrogen enhances the inhibitory effect of an angiotensin II type-1 ( AT1 ) receptor blocker ( ARB ) , olmesartan , on atherosclerosis , focusing on oxidative stress using apolipoprotein E knockout mice ( ApoEKO ) .
	manualset3
160141	6	411705	7	NULL	NULL	0	NULL	olmesartan	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study explored the possibility that estrogen enhances the inhibitory effect of an angiotensin II type-1 ( AT1 ) receptor blocker ( ARB ) , olmesartan , on atherosclerosis , focusing on oxidative stress using apolipoprotein E knockout mice ( ApoEKO ) .
	manualset3
160142	7	411705	7	NULL	NULL	0	NULL	 atherosclerosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study explored the possibility that estrogen enhances the inhibitory effect of an angiotensin II type-1 ( AT1 ) receptor blocker ( ARB ) , olmesartan , on atherosclerosis , focusing on oxidative stress using apolipoprotein E knockout mice ( ApoEKO ) .
	manualset3
160143	8	411705	7	NULL	NULL	0	NULL	oxidative stress	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study explored the possibility that estrogen enhances the inhibitory effect of an angiotensin II type-1 ( AT1 ) receptor blocker ( ARB ) , olmesartan , on atherosclerosis , focusing on oxidative stress using apolipoprotein E knockout mice ( ApoEKO ) .
	manualset3
160144	9	411705	7	NULL	NULL	0	NULL	apolipoprotein E knockout mice ( ApoEKO )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study explored the possibility that estrogen enhances the inhibitory effect of an angiotensin II type-1 ( AT1 ) receptor blocker ( ARB ) , olmesartan , on atherosclerosis , focusing on oxidative stress using apolipoprotein E knockout mice ( ApoEKO ) .
	manualset3
160145	1	411706	7	NULL	NULL	0	NULL	APSTs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	APSTs with microinvasion are more common than earlier appreciated .
	manualset3
160146	2	411706	7	NULL	NULL	0	NULL	microinvasion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	APSTs with microinvasion are more common than earlier appreciated .
	manualset3
160147	1	411707	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study has characterized the cellular and temporal localization of the phospholipase D2 ( PLD2 ) protein in the embryonic rat brain , using immunohistochemistry .
	manualset3
160148	2	411707	7	NULL	NULL	0	NULL	 cellular localization 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study has characterized the cellular and temporal localization of the phospholipase D2 ( PLD2 ) protein in the embryonic rat brain , using immunohistochemistry .
	manualset3
160149	3	411707	7	NULL	NULL	0	NULL	temporal localization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study has characterized the cellular and temporal localization of the phospholipase D2 ( PLD2 ) protein in the embryonic rat brain , using immunohistochemistry .
	manualset3
160150	4	411707	7	NULL	NULL	0	NULL	phospholipase D2 ( PLD2 ) protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study has characterized the cellular and temporal localization of the phospholipase D2 ( PLD2 ) protein in the embryonic rat brain , using immunohistochemistry .
	manualset3
160151	5	411707	7	NULL	NULL	0	NULL	embryonic rat brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study has characterized the cellular and temporal localization of the phospholipase D2 ( PLD2 ) protein in the embryonic rat brain , using immunohistochemistry .
	manualset3
160152	6	411707	7	NULL	NULL	0	NULL	 immunohistochemistry 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study has characterized the cellular and temporal localization of the phospholipase D2 ( PLD2 ) protein in the embryonic rat brain , using immunohistochemistry .
	manualset3
160153	1	411708	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study indicates that , during a certain period of the growth transition , twice as much beta subunit is synthesized as beta ' subunit and the overproduced beta subunit accumulates as the assembly intermediate alpha 2 beta complex , which is rapidly and preferentially degraded .
	manualset3
160154	2	411708	7	NULL	NULL	0	NULL	period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study indicates that , during a certain period of the growth transition , twice as much beta subunit is synthesized as beta ' subunit and the overproduced beta subunit accumulates as the assembly intermediate alpha 2 beta complex , which is rapidly and preferentially degraded .
	manualset3
160155	3	411708	7	NULL	NULL	0	NULL	growth transition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study indicates that , during a certain period of the growth transition , twice as much beta subunit is synthesized as beta ' subunit and the overproduced beta subunit accumulates as the assembly intermediate alpha 2 beta complex , which is rapidly and preferentially degraded .
	manualset3
160156	4	411708	7	NULL	NULL	0	NULL	beta subunit	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study indicates that , during a certain period of the growth transition , twice as much beta subunit is synthesized as beta ' subunit and the overproduced beta subunit accumulates as the assembly intermediate alpha 2 beta complex , which is rapidly and preferentially degraded .
	manualset3
160157	5	411708	7	NULL	NULL	0	NULL	beta ' subunit	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study indicates that , during a certain period of the growth transition , twice as much beta subunit is synthesized as beta ' subunit and the overproduced beta subunit accumulates as the assembly intermediate alpha 2 beta complex , which is rapidly and preferentially degraded .
	manualset3
160158	6	411708	7	NULL	NULL	0	NULL	beta subunit	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study indicates that , during a certain period of the growth transition , twice as much beta subunit is synthesized as beta ' subunit and the overproduced beta subunit accumulates as the assembly intermediate alpha 2 beta complex , which is rapidly and preferentially degraded .
	manualset3
160159	7	411708	7	NULL	NULL	NULL	NULL	assembly	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present study indicates that , during a certain period of the growth transition , twice as much beta subunit is synthesized as beta ' subunit and the overproduced beta subunit accumulates as the assembly intermediate alpha 2 beta complex , which is rapidly and preferentially degraded .
	manualset3
160160	8	411708	7	NULL	NULL	0	NULL	alpha 2 beta complex	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study indicates that , during a certain period of the growth transition , twice as much beta subunit is synthesized as beta ' subunit and the overproduced beta subunit accumulates as the assembly intermediate alpha 2 beta complex , which is rapidly and preferentially degraded .
	manualset3
160161	1	411709	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study indicates that C-band heteromorphisms may play some role in the development of malignancy of the uterine cervix .
	manualset3
160162	2	411709	7	NULL	NULL	0	NULL	C-band heteromorphisms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study indicates that C-band heteromorphisms may play some role in the development of malignancy of the uterine cervix .
	manualset3
160163	3	411709	7	NULL	NULL	0	NULL	 role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study indicates that C-band heteromorphisms may play some role in the development of malignancy of the uterine cervix .
	manualset3
160164	4	411709	7	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study indicates that C-band heteromorphisms may play some role in the development of malignancy of the uterine cervix .
	manualset3
160165	5	411709	7	NULL	NULL	0	NULL	 malignancy of the uterine cervix	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study indicates that C-band heteromorphisms may play some role in the development of malignancy of the uterine cervix .
	manualset3
160166	1	411710	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study investigated the effects of a preparation of a gamma-tocopherol-rich mixture of tocopherols ( gamma-TmT ) on chemically induced lung tumorigenesis in female A/J mice and the growth of H1299 human lung cancer cell xenograft tumors .
	manualset3
160167	2	411710	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study investigated the effects of a preparation of a gamma-tocopherol-rich mixture of tocopherols ( gamma-TmT ) on chemically induced lung tumorigenesis in female A/J mice and the growth of H1299 human lung cancer cell xenograft tumors .
	manualset3
160168	3	411710	7	NULL	NULL	0	NULL	preparation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study investigated the effects of a preparation of a gamma-tocopherol-rich mixture of tocopherols ( gamma-TmT ) on chemically induced lung tumorigenesis in female A/J mice and the growth of H1299 human lung cancer cell xenograft tumors .
	manualset3
160169	4	411710	7	NULL	NULL	0	NULL	gamma-tocopherol-rich mixture of tocopherols ( gamma-TmT )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study investigated the effects of a preparation of a gamma-tocopherol-rich mixture of tocopherols ( gamma-TmT ) on chemically induced lung tumorigenesis in female A/J mice and the growth of H1299 human lung cancer cell xenograft tumors .
	manualset3
160170	5	411710	7	NULL	NULL	0	NULL	chemically induced lung tumorigenesis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study investigated the effects of a preparation of a gamma-tocopherol-rich mixture of tocopherols ( gamma-TmT ) on chemically induced lung tumorigenesis in female A/J mice and the growth of H1299 human lung cancer cell xenograft tumors .
	manualset3
160171	6	411710	7	NULL	NULL	0	NULL	 female A/J mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study investigated the effects of a preparation of a gamma-tocopherol-rich mixture of tocopherols ( gamma-TmT ) on chemically induced lung tumorigenesis in female A/J mice and the growth of H1299 human lung cancer cell xenograft tumors .
	manualset3
160172	7	411710	7	NULL	NULL	NULL	NULL	 growth  	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present study investigated the effects of a preparation of a gamma-tocopherol-rich mixture of tocopherols ( gamma-TmT ) on chemically induced lung tumorigenesis in female A/J mice and the growth of H1299 human lung cancer cell xenograft tumors .
	manualset3
160173	8	411710	7	NULL	NULL	NULL	NULL	H1299 human lung cancer cell xenograft tumors	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present study investigated the effects of a preparation of a gamma-tocopherol-rich mixture of tocopherols ( gamma-TmT ) on chemically induced lung tumorigenesis in female A/J mice and the growth of H1299 human lung cancer cell xenograft tumors .
	manualset3
160174	1	411711	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study investigated the proximal constraints that determine perceptual unit formation under minimal stimulus conditions .
	manualset3
160175	2	411711	7	NULL	NULL	0	NULL	proximal constraints 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study investigated the proximal constraints that determine perceptual unit formation under minimal stimulus conditions .
	manualset3
160176	3	411711	7	NULL	NULL	0	NULL	perceptual unit formation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study investigated the proximal constraints that determine perceptual unit formation under minimal stimulus conditions .
	manualset3
160177	4	411711	7	NULL	NULL	0	NULL	minimal stimulus conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study investigated the proximal constraints that determine perceptual unit formation under minimal stimulus conditions .
	manualset3
160178	1	411712	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study involved in-vitro and in-vivo investigations of whether Sr might first be an inhibitor of adipogenesis , thus explaining late osteoblastogenesis .
	manualset3
160179	2	411712	7	NULL	NULL	0	NULL	 in-vitro investigations 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study involved in-vitro and in-vivo investigations of whether Sr might first be an inhibitor of adipogenesis , thus explaining late osteoblastogenesis .
	manualset3
160180	3	411712	7	NULL	NULL	0	NULL	in-vivo investigations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study involved in-vitro and in-vivo investigations of whether Sr might first be an inhibitor of adipogenesis , thus explaining late osteoblastogenesis .
	manualset3
160181	4	411712	7	NULL	NULL	0	NULL	 Sr	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study involved in-vitro and in-vivo investigations of whether Sr might first be an inhibitor of adipogenesis , thus explaining late osteoblastogenesis .
	manualset3
160182	5	411712	7	NULL	NULL	NULL	NULL	 inhibitor	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present study involved in-vitro and in-vivo investigations of whether Sr might first be an inhibitor of adipogenesis , thus explaining late osteoblastogenesis .
	manualset3
160183	6	411712	7	NULL	NULL	0	NULL	adipogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study involved in-vitro and in-vivo investigations of whether Sr might first be an inhibitor of adipogenesis , thus explaining late osteoblastogenesis .
	manualset3
160184	7	411712	7	NULL	NULL	0	NULL	late osteoblastogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study involved in-vitro and in-vivo investigations of whether Sr might first be an inhibitor of adipogenesis , thus explaining late osteoblastogenesis .
	manualset3
160185	1	411713	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study is the first report elucidating the chemical structures and changes in individual concentrations in rat plasma of glucuronides derived from orally administered hesperidin .
	manualset3
160186	2	411713	7	NULL	NULL	0	NULL	first report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study is the first report elucidating the chemical structures and changes in individual concentrations in rat plasma of glucuronides derived from orally administered hesperidin .
	manualset3
160187	3	411713	7	NULL	NULL	0	NULL	chemical structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study is the first report elucidating the chemical structures and changes in individual concentrations in rat plasma of glucuronides derived from orally administered hesperidin .
	manualset3
160188	4	411713	7	NULL	NULL	0	NULL	concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study is the first report elucidating the chemical structures and changes in individual concentrations in rat plasma of glucuronides derived from orally administered hesperidin .
	manualset3
160189	5	411713	7	NULL	NULL	0	NULL	rat plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study is the first report elucidating the chemical structures and changes in individual concentrations in rat plasma of glucuronides derived from orally administered hesperidin .
	manualset3
160190	6	411713	7	NULL	NULL	0	NULL	glucuronides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study is the first report elucidating the chemical structures and changes in individual concentrations in rat plasma of glucuronides derived from orally administered hesperidin .
	manualset3
160191	7	411713	7	NULL	NULL	0	NULL	hesperidin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study is the first report elucidating the chemical structures and changes in individual concentrations in rat plasma of glucuronides derived from orally administered hesperidin .
	manualset3
160192	1	411714	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study provides evidence that Cd transport by N. diversicolor was mediated mainly through lanthanum - sensitive Ca ion channels and accumulated by SH-containing compounds .
	manualset3
160193	2	411714	7	NULL	NULL	0	NULL	Cd transport 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study provides evidence that Cd transport by N. diversicolor was mediated mainly through lanthanum - sensitive Ca ion channels and accumulated by SH-containing compounds .
	manualset3
160194	3	411714	7	NULL	NULL	0	NULL	N. diversicolor	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study provides evidence that Cd transport by N. diversicolor was mediated mainly through lanthanum - sensitive Ca ion channels and accumulated by SH-containing compounds .
	manualset3
160195	4	411714	7	NULL	NULL	0	NULL	 lanthanum - sensitive Ca ion channels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study provides evidence that Cd transport by N. diversicolor was mediated mainly through lanthanum - sensitive Ca ion channels and accumulated by SH-containing compounds .
	manualset3
160196	5	411714	7	NULL	NULL	0	NULL	SH-containing compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study provides evidence that Cd transport by N. diversicolor was mediated mainly through lanthanum - sensitive Ca ion channels and accumulated by SH-containing compounds .
	manualset3
160962	6	411714	7	NULL	NULL	0	NULL	evidence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study provides evidence that Cd transport by N. diversicolor was mediated mainly through lanthanum - sensitive Ca ion channels and accumulated by SH-containing compounds .
	manualset3
160197	1	411715	7	NULL	NULL	NULL	NULL	AQP10	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	AQP10 is localized on the apical compartment of the intestinal epithelium called the glycocalyx while AQP3 is selectively targeted to the basolateral membrane .
	manualset3
160198	2	411715	7	NULL	NULL	0	NULL	 apical compartment	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	AQP10 is localized on the apical compartment of the intestinal epithelium called the glycocalyx while AQP3 is selectively targeted to the basolateral membrane .
	manualset3
160199	3	411715	7	NULL	NULL	0	NULL	 intestinal epithelium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	AQP10 is localized on the apical compartment of the intestinal epithelium called the glycocalyx while AQP3 is selectively targeted to the basolateral membrane .
	manualset3
160200	4	411715	7	NULL	NULL	0	NULL	glycocalyx	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	AQP10 is localized on the apical compartment of the intestinal epithelium called the glycocalyx while AQP3 is selectively targeted to the basolateral membrane .
	manualset3
160201	5	411715	7	NULL	NULL	0	NULL	AQP3	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	AQP10 is localized on the apical compartment of the intestinal epithelium called the glycocalyx while AQP3 is selectively targeted to the basolateral membrane .
	manualset3
160202	6	411715	7	NULL	NULL	0	NULL	basolateral membrane	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	AQP10 is localized on the apical compartment of the intestinal epithelium called the glycocalyx while AQP3 is selectively targeted to the basolateral membrane .
	manualset3
160203	1	411716	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study shows that this difference in the toxicity most likely can not be attributed to maleic acid , furan , furfural , furfuryl alcohol , or 2-furoic acid .
	manualset3
160204	2	411716	7	NULL	NULL	0	NULL	toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study shows that this difference in the toxicity most likely can not be attributed to maleic acid , furan , furfural , furfuryl alcohol , or 2-furoic acid .
	manualset3
160205	3	411716	7	NULL	NULL	0	NULL	maleic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study shows that this difference in the toxicity most likely can not be attributed to maleic acid , furan , furfural , furfuryl alcohol , or 2-furoic acid .
	manualset3
160206	4	411716	7	NULL	NULL	0	NULL	furan	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study shows that this difference in the toxicity most likely can not be attributed to maleic acid , furan , furfural , furfuryl alcohol , or 2-furoic acid .
	manualset3
160207	5	411716	7	NULL	NULL	0	NULL	furfural	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study shows that this difference in the toxicity most likely can not be attributed to maleic acid , furan , furfural , furfuryl alcohol , or 2-furoic acid .
	manualset3
160208	6	411716	7	NULL	NULL	0	NULL	furfuryl alcohol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study shows that this difference in the toxicity most likely can not be attributed to maleic acid , furan , furfural , furfuryl alcohol , or 2-furoic acid .
	manualset3
160209	7	411716	7	NULL	NULL	0	NULL	2-furoic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study shows that this difference in the toxicity most likely can not be attributed to maleic acid , furan , furfural , furfuryl alcohol , or 2-furoic acid .
	manualset3
169192	8	411716	7	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study shows that this difference in the toxicity most likely can not be attributed to maleic acid , furan , furfural , furfuryl alcohol , or 2-furoic acid .
	manualset3
160210	1	411717	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study suggests that the ghrelin precursor polymorphism may not confer a susceptibility to the development of methamphetamine dependence in the Korean population .
	manualset3
160211	2	411717	7	NULL	NULL	NULL	NULL	ghrelin precursor polymorphism	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present study suggests that the ghrelin precursor polymorphism may not confer a susceptibility to the development of methamphetamine dependence in the Korean population .
	manualset3
160212	3	411717	7	NULL	NULL	NULL	NULL	development	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present study suggests that the ghrelin precursor polymorphism may not confer a susceptibility to the development of methamphetamine dependence in the Korean population .
	manualset3
160213	4	411717	7	NULL	NULL	0	NULL	methamphetamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study suggests that the ghrelin precursor polymorphism may not confer a susceptibility to the development of methamphetamine dependence in the Korean population .
	manualset3
160214	5	411717	7	NULL	NULL	0	NULL	Korean population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study suggests that the ghrelin precursor polymorphism may not confer a susceptibility to the development of methamphetamine dependence in the Korean population .
	manualset3
169193	6	411717	7	NULL	NULL	0	NULL	susceptibility	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study suggests that the ghrelin precursor polymorphism may not confer a susceptibility to the development of methamphetamine dependence in the Korean population .
	manualset3
160215	1	411718	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was conducted to demonstrate how high-dose thyroxin administration for one week affected oxidative damage formed in experimental hypothyroidism .
	manualset3
160216	2	411718	7	NULL	NULL	0	NULL	high-dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was conducted to demonstrate how high-dose thyroxin administration for one week affected oxidative damage formed in experimental hypothyroidism .
	manualset3
160217	3	411718	7	NULL	NULL	0	NULL	thyroxin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was conducted to demonstrate how high-dose thyroxin administration for one week affected oxidative damage formed in experimental hypothyroidism .
	manualset3
160218	4	411718	7	NULL	NULL	0	NULL	administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was conducted to demonstrate how high-dose thyroxin administration for one week affected oxidative damage formed in experimental hypothyroidism .
	manualset3
160219	5	411718	7	NULL	NULL	0	NULL	one week	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was conducted to demonstrate how high-dose thyroxin administration for one week affected oxidative damage formed in experimental hypothyroidism .
	manualset3
160220	6	411718	7	NULL	NULL	0	NULL	oxidative damage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was conducted to demonstrate how high-dose thyroxin administration for one week affected oxidative damage formed in experimental hypothyroidism .
	manualset3
160221	7	411718	7	NULL	NULL	0	NULL	experimental hypothyroidism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was conducted to demonstrate how high-dose thyroxin administration for one week affected oxidative damage formed in experimental hypothyroidism .
	manualset3
160222	1	411719	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was design to examine the effect of tautomerism upon the CoMFA results .
	manualset3
160223	2	411719	7	NULL	NULL	0	NULL	tautomerism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was design to examine the effect of tautomerism upon the CoMFA results .
	manualset3
160224	3	411719	7	NULL	NULL	0	NULL	CoMFA results	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was design to examine the effect of tautomerism upon the CoMFA results .
	manualset3
160225	1	411720	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to characterize the cross-talk of parathyroid hormone ( PTH ) - responsive dual signal transduction systems ( cAMP-dependent protein kinase ( PKA ) and calcium/protein kinase C ( PKC ) ) and its participation in PTH-induced homologous desensitization of intracellular calcium ( ( Ca2 + ) i ) in osteoblastic UMR-106 cells .
	manualset3
160226	2	411720	7	NULL	NULL	NULL	NULL	cross-talk 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present study was designed to characterize the cross-talk of parathyroid hormone ( PTH ) - responsive dual signal transduction systems ( cAMP-dependent protein kinase ( PKA ) and calcium/protein kinase C ( PKC ) ) and its participation in PTH-induced homologous desensitization of intracellular calcium ( ( Ca2 + ) i ) in osteoblastic UMR-106 cells .
	manualset3
160227	3	411720	7	NULL	NULL	0	NULL	parathyroid hormone ( PTH ) - responsive dual signal transduction systems	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to characterize the cross-talk of parathyroid hormone ( PTH ) - responsive dual signal transduction systems ( cAMP-dependent protein kinase ( PKA ) and calcium/protein kinase C ( PKC ) ) and its participation in PTH-induced homologous desensitization of intracellular calcium ( ( Ca2 + ) i ) in osteoblastic UMR-106 cells .
	manualset3
160228	4	411720	7	NULL	NULL	0	NULL	cAMP-dependent protein kinase ( PKA )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to characterize the cross-talk of parathyroid hormone ( PTH ) - responsive dual signal transduction systems ( cAMP-dependent protein kinase ( PKA ) and calcium/protein kinase C ( PKC ) ) and its participation in PTH-induced homologous desensitization of intracellular calcium ( ( Ca2 + ) i ) in osteoblastic UMR-106 cells .
	manualset3
160229	5	411720	7	NULL	NULL	0	NULL	calcium/protein kinase C ( PKC 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to characterize the cross-talk of parathyroid hormone ( PTH ) - responsive dual signal transduction systems ( cAMP-dependent protein kinase ( PKA ) and calcium/protein kinase C ( PKC ) ) and its participation in PTH-induced homologous desensitization of intracellular calcium ( ( Ca2 + ) i ) in osteoblastic UMR-106 cells .
	manualset3
160230	6	411720	7	NULL	NULL	0	NULL	participation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to characterize the cross-talk of parathyroid hormone ( PTH ) - responsive dual signal transduction systems ( cAMP-dependent protein kinase ( PKA ) and calcium/protein kinase C ( PKC ) ) and its participation in PTH-induced homologous desensitization of intracellular calcium ( ( Ca2 + ) i ) in osteoblastic UMR-106 cells .
	manualset3
160231	7	411720	7	NULL	NULL	0	NULL	PTH-induced homologous desensitization of intracellular calcium ( ( Ca2 + ) i )	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to characterize the cross-talk of parathyroid hormone ( PTH ) - responsive dual signal transduction systems ( cAMP-dependent protein kinase ( PKA ) and calcium/protein kinase C ( PKC ) ) and its participation in PTH-induced homologous desensitization of intracellular calcium ( ( Ca2 + ) i ) in osteoblastic UMR-106 cells .
	manualset3
160232	8	411720	7	NULL	NULL	0	NULL	osteoblastic UMR-106 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to characterize the cross-talk of parathyroid hormone ( PTH ) - responsive dual signal transduction systems ( cAMP-dependent protein kinase ( PKA ) and calcium/protein kinase C ( PKC ) ) and its participation in PTH-induced homologous desensitization of intracellular calcium ( ( Ca2 + ) i ) in osteoblastic UMR-106 cells .
	manualset3
160233	1	411721	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to examine the role of adenosine receptors in the short-term social memory of rats using the social recognition paradigm .
	manualset3
160234	2	411721	7	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to examine the role of adenosine receptors in the short-term social memory of rats using the social recognition paradigm .
	manualset3
160235	3	411721	7	NULL	NULL	0	NULL	adenosine receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to examine the role of adenosine receptors in the short-term social memory of rats using the social recognition paradigm .
	manualset3
160236	4	411721	7	NULL	NULL	0	NULL	short-term social memory 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to examine the role of adenosine receptors in the short-term social memory of rats using the social recognition paradigm .
	manualset3
160237	5	411721	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to examine the role of adenosine receptors in the short-term social memory of rats using the social recognition paradigm .
	manualset3
160238	6	411721	7	NULL	NULL	NULL	NULL	social recognition paradigm	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present study was designed to examine the role of adenosine receptors in the short-term social memory of rats using the social recognition paradigm .
	manualset3
160239	1	411722	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to examine whether gastrin hypersecretion in response to treatment with antisecretory drugs induces an inflammatory response that could promote mucosal atrophy .
	manualset3
160240	2	411722	7	NULL	NULL	0	NULL	 gastrin hypersecretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to examine whether gastrin hypersecretion in response to treatment with antisecretory drugs induces an inflammatory response that could promote mucosal atrophy .
	manualset3
160241	3	411722	7	NULL	NULL	0	NULL	 response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to examine whether gastrin hypersecretion in response to treatment with antisecretory drugs induces an inflammatory response that could promote mucosal atrophy .
	manualset3
160242	4	411722	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to examine whether gastrin hypersecretion in response to treatment with antisecretory drugs induces an inflammatory response that could promote mucosal atrophy .
	manualset3
160243	5	411722	7	NULL	NULL	0	NULL	antisecretory drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to examine whether gastrin hypersecretion in response to treatment with antisecretory drugs induces an inflammatory response that could promote mucosal atrophy .
	manualset3
160244	6	411722	7	NULL	NULL	0	NULL	 inflammatory response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to examine whether gastrin hypersecretion in response to treatment with antisecretory drugs induces an inflammatory response that could promote mucosal atrophy .
	manualset3
160245	7	411722	7	NULL	NULL	0	NULL	mucosal atrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to examine whether gastrin hypersecretion in response to treatment with antisecretory drugs induces an inflammatory response that could promote mucosal atrophy .
	manualset3
160246	1	411723	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to examine whether naturally occurring CD4 ( + ) CD25 ( + ) Tregs isolated from murine spleens expressed TIPE2 by the use of Western blot and reverse transcription-polymerase chain reaction ( RT-PCR ) .
	manualset3
160247	2	411723	7	NULL	NULL	0	NULL	CD4 ( + ) CD25 ( + ) Tregs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to examine whether naturally occurring CD4 ( + ) CD25 ( + ) Tregs isolated from murine spleens expressed TIPE2 by the use of Western blot and reverse transcription-polymerase chain reaction ( RT-PCR ) .
	manualset3
160248	3	411723	7	NULL	NULL	0	NULL	murine spleens 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to examine whether naturally occurring CD4 ( + ) CD25 ( + ) Tregs isolated from murine spleens expressed TIPE2 by the use of Western blot and reverse transcription-polymerase chain reaction ( RT-PCR ) .
	manualset3
160249	4	411723	7	NULL	NULL	0	NULL	TIPE2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to examine whether naturally occurring CD4 ( + ) CD25 ( + ) Tregs isolated from murine spleens expressed TIPE2 by the use of Western blot and reverse transcription-polymerase chain reaction ( RT-PCR ) .
	manualset3
160250	5	411723	7	NULL	NULL	0	NULL	Western blot 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to examine whether naturally occurring CD4 ( + ) CD25 ( + ) Tregs isolated from murine spleens expressed TIPE2 by the use of Western blot and reverse transcription-polymerase chain reaction ( RT-PCR ) .
	manualset3
160251	6	411723	7	NULL	NULL	0	NULL	reverse transcription-polymerase chain reaction ( RT-PCR ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to examine whether naturally occurring CD4 ( + ) CD25 ( + ) Tregs isolated from murine spleens expressed TIPE2 by the use of Western blot and reverse transcription-polymerase chain reaction ( RT-PCR ) .
	manualset3
160252	1	411724	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to investigate the effect of sildenafil on learning and memory in mice using elevated plus maze .
	manualset3
160253	2	411724	7	NULL	NULL	0	NULL	sildenafil 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to investigate the effect of sildenafil on learning and memory in mice using elevated plus maze .
	manualset3
160254	3	411724	7	NULL	NULL	0	NULL	learning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to investigate the effect of sildenafil on learning and memory in mice using elevated plus maze .
	manualset3
160255	4	411724	7	NULL	NULL	0	NULL	memory	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to investigate the effect of sildenafil on learning and memory in mice using elevated plus maze .
	manualset3
160256	5	411724	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to investigate the effect of sildenafil on learning and memory in mice using elevated plus maze .
	manualset3
160257	6	411724	7	NULL	NULL	0	NULL	elevated plus maze	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to investigate the effect of sildenafil on learning and memory in mice using elevated plus maze .
	manualset3
169194	7	411724	7	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to investigate the effect of sildenafil on learning and memory in mice using elevated plus maze .
	manualset3
160258	1	411725	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to investigate the relative acute toxicity of acid mine drainage ( AMD ) water column and sediments to a single test organism ( Daphnia magna ) and to determine which abiotic factors were the best indicators of toxicity in this system .
	manualset3
160259	2	411725	7	NULL	NULL	NULL	NULL	 relative acute toxicity 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present study was designed to investigate the relative acute toxicity of acid mine drainage ( AMD ) water column and sediments to a single test organism ( Daphnia magna ) and to determine which abiotic factors were the best indicators of toxicity in this system .
	manualset3
160260	3	411725	7	NULL	NULL	0	NULL	acid mine drainage ( AMD ) water column	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to investigate the relative acute toxicity of acid mine drainage ( AMD ) water column and sediments to a single test organism ( Daphnia magna ) and to determine which abiotic factors were the best indicators of toxicity in this system .
	manualset3
160261	4	411725	7	NULL	NULL	0	NULL	sediments	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to investigate the relative acute toxicity of acid mine drainage ( AMD ) water column and sediments to a single test organism ( Daphnia magna ) and to determine which abiotic factors were the best indicators of toxicity in this system .
	manualset3
160262	5	411725	7	NULL	NULL	0	NULL	single test organism 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to investigate the relative acute toxicity of acid mine drainage ( AMD ) water column and sediments to a single test organism ( Daphnia magna ) and to determine which abiotic factors were the best indicators of toxicity in this system .
	manualset3
160263	6	411725	7	NULL	NULL	0	NULL	Daphnia magna	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to investigate the relative acute toxicity of acid mine drainage ( AMD ) water column and sediments to a single test organism ( Daphnia magna ) and to determine which abiotic factors were the best indicators of toxicity in this system .
	manualset3
160264	7	411725	7	NULL	NULL	0	NULL	abiotic factors	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to investigate the relative acute toxicity of acid mine drainage ( AMD ) water column and sediments to a single test organism ( Daphnia magna ) and to determine which abiotic factors were the best indicators of toxicity in this system .
	manualset3
160265	8	411725	7	NULL	NULL	NULL	NULL	 indicators	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present study was designed to investigate the relative acute toxicity of acid mine drainage ( AMD ) water column and sediments to a single test organism ( Daphnia magna ) and to determine which abiotic factors were the best indicators of toxicity in this system .
	manualset3
160266	9	411725	7	NULL	NULL	0	NULL	toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to investigate the relative acute toxicity of acid mine drainage ( AMD ) water column and sediments to a single test organism ( Daphnia magna ) and to determine which abiotic factors were the best indicators of toxicity in this system .
	manualset3
160267	10	411725	7	NULL	NULL	0	NULL	system 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to investigate the relative acute toxicity of acid mine drainage ( AMD ) water column and sediments to a single test organism ( Daphnia magna ) and to determine which abiotic factors were the best indicators of toxicity in this system .
	manualset3
160268	1	411726	7	NULL	NULL	0	NULL	Clinical statistics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical statistics on the indication for the cesarean section in the decade from 1947 to 1956 ) .
	manualset3
160269	2	411726	7	NULL	NULL	0	NULL	 indication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical statistics on the indication for the cesarean section in the decade from 1947 to 1956 ) .
	manualset3
160270	3	411726	7	NULL	NULL	0	NULL	cesarean section	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical statistics on the indication for the cesarean section in the decade from 1947 to 1956 ) .
	manualset3
160271	4	411726	7	NULL	NULL	0	NULL	decade	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical statistics on the indication for the cesarean section in the decade from 1947 to 1956 ) .
	manualset3
160272	5	411726	7	NULL	NULL	0	NULL	1947 to 1956 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical statistics on the indication for the cesarean section in the decade from 1947 to 1956 ) .
	manualset3
160273	1	411727	7	NULL	NULL	0	NULL	ARBs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	ARBs prevent stroke incidence by blocking the angiotensin II ( AII ) , AT1 receptors preventing brain ischemia and allowing AII to stimulate the unoccupied AT2 receptors , which improve brain ischemia .
	manualset3
160274	2	411727	7	NULL	NULL	0	NULL	stroke	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	ARBs prevent stroke incidence by blocking the angiotensin II ( AII ) , AT1 receptors preventing brain ischemia and allowing AII to stimulate the unoccupied AT2 receptors , which improve brain ischemia .
	manualset3
160275	3	411727	7	NULL	NULL	0	NULL	angiotensin II ( AII ) receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	ARBs prevent stroke incidence by blocking the angiotensin II ( AII ) , AT1 receptors preventing brain ischemia and allowing AII to stimulate the unoccupied AT2 receptors , which improve brain ischemia .
	manualset3
160276	4	411727	7	NULL	NULL	0	NULL	AT1 receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	ARBs prevent stroke incidence by blocking the angiotensin II ( AII ) , AT1 receptors preventing brain ischemia and allowing AII to stimulate the unoccupied AT2 receptors , which improve brain ischemia .
	manualset3
160277	5	411727	7	NULL	NULL	0	NULL	brain ischemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	ARBs prevent stroke incidence by blocking the angiotensin II ( AII ) , AT1 receptors preventing brain ischemia and allowing AII to stimulate the unoccupied AT2 receptors , which improve brain ischemia .
	manualset3
160278	6	411727	7	NULL	NULL	0	NULL	AII	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	ARBs prevent stroke incidence by blocking the angiotensin II ( AII ) , AT1 receptors preventing brain ischemia and allowing AII to stimulate the unoccupied AT2 receptors , which improve brain ischemia .
	manualset3
160279	7	411727	7	NULL	NULL	0	NULL	unoccupied AT2 receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	ARBs prevent stroke incidence by blocking the angiotensin II ( AII ) , AT1 receptors preventing brain ischemia and allowing AII to stimulate the unoccupied AT2 receptors , which improve brain ischemia .
	manualset3
160280	8	411727	7	NULL	NULL	0	NULL	brain ischemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	ARBs prevent stroke incidence by blocking the angiotensin II ( AII ) , AT1 receptors preventing brain ischemia and allowing AII to stimulate the unoccupied AT2 receptors , which improve brain ischemia .
	manualset3
160281	1	411728	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to test the hypothesis , based on observations of decreased apolipoprotein B ( ApoB ) synthesis and secretion in vitro , that ACTH administration inhibits the postprandial output of ApoB in man .
	manualset3
160282	2	411728	7	NULL	NULL	0	NULL	hypothesis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to test the hypothesis , based on observations of decreased apolipoprotein B ( ApoB ) synthesis and secretion in vitro , that ACTH administration inhibits the postprandial output of ApoB in man .
	manualset3
160283	3	411728	7	NULL	NULL	0	NULL	apolipoprotein B ( ApoB ) synthesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to test the hypothesis , based on observations of decreased apolipoprotein B ( ApoB ) synthesis and secretion in vitro , that ACTH administration inhibits the postprandial output of ApoB in man .
	manualset3
160284	4	411728	7	NULL	NULL	0	NULL	 secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to test the hypothesis , based on observations of decreased apolipoprotein B ( ApoB ) synthesis and secretion in vitro , that ACTH administration inhibits the postprandial output of ApoB in man .
	manualset3
160285	5	411728	7	NULL	NULL	0	NULL	ACTH administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to test the hypothesis , based on observations of decreased apolipoprotein B ( ApoB ) synthesis and secretion in vitro , that ACTH administration inhibits the postprandial output of ApoB in man .
	manualset3
160286	6	411728	7	NULL	NULL	0	NULL	postprandial output 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to test the hypothesis , based on observations of decreased apolipoprotein B ( ApoB ) synthesis and secretion in vitro , that ACTH administration inhibits the postprandial output of ApoB in man .
	manualset3
160287	7	411728	7	NULL	NULL	0	NULL	ApoB 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to test the hypothesis , based on observations of decreased apolipoprotein B ( ApoB ) synthesis and secretion in vitro , that ACTH administration inhibits the postprandial output of ApoB in man .
	manualset3
160288	8	411728	7	NULL	NULL	0	NULL	 man	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was designed to test the hypothesis , based on observations of decreased apolipoprotein B ( ApoB ) synthesis and secretion in vitro , that ACTH administration inhibits the postprandial output of ApoB in man .
	manualset3
160289	1	411729	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to confirm the phenomenon of infection exclusion of A. marginale genotypes in a tick vector , Dermacentor variabilis .
	manualset3
160290	2	411729	7	NULL	NULL	NULL	NULL	phenomenon 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to confirm the phenomenon of infection exclusion of A. marginale genotypes in a tick vector , Dermacentor variabilis .
	manualset3
160291	3	411729	7	NULL	NULL	0	NULL	infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to confirm the phenomenon of infection exclusion of A. marginale genotypes in a tick vector , Dermacentor variabilis .
	manualset3
160292	5	411729	7	NULL	NULL	NULL	NULL	A. marginale genotypes	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to confirm the phenomenon of infection exclusion of A. marginale genotypes in a tick vector , Dermacentor variabilis .
	manualset3
160293	4	411729	7	NULL	NULL	0	NULL	exclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to confirm the phenomenon of infection exclusion of A. marginale genotypes in a tick vector , Dermacentor variabilis .
	manualset3
160294	6	411729	7	NULL	NULL	0	NULL	tick vector	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to confirm the phenomenon of infection exclusion of A. marginale genotypes in a tick vector , Dermacentor variabilis .
	manualset3
160295	7	411729	7	NULL	NULL	0	NULL	Dermacentor variabilis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to confirm the phenomenon of infection exclusion of A. marginale genotypes in a tick vector , Dermacentor variabilis .
	manualset3
160296	1	411730	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to determine whether oltipraz can also influence expression of genes encoding antioxidant enzymes .
	manualset3
160297	2	411730	7	NULL	NULL	0	NULL	oltipraz	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to determine whether oltipraz can also influence expression of genes encoding antioxidant enzymes .
	manualset3
160298	3	411730	7	NULL	NULL	0	NULL	expression of genes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to determine whether oltipraz can also influence expression of genes encoding antioxidant enzymes .
	manualset3
160299	4	411730	7	NULL	NULL	0	NULL	antioxidant enzymes	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to determine whether oltipraz can also influence expression of genes encoding antioxidant enzymes .
	manualset3
160300	1	411731	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to estimate the difference in interaction of human and rat factors with human APC and to assess the cause of the species specificity .
	manualset3
160301	2	411731	7	NULL	NULL	0	NULL	interaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to estimate the difference in interaction of human and rat factors with human APC and to assess the cause of the species specificity .
	manualset3
160302	3	411731	7	NULL	NULL	0	NULL	human factors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to estimate the difference in interaction of human and rat factors with human APC and to assess the cause of the species specificity .
	manualset3
160303	4	411731	7	NULL	NULL	0	NULL	 rat factors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to estimate the difference in interaction of human and rat factors with human APC and to assess the cause of the species specificity .
	manualset3
160304	5	411731	7	NULL	NULL	0	NULL	human APC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to estimate the difference in interaction of human and rat factors with human APC and to assess the cause of the species specificity .
	manualset3
160305	7	411731	7	NULL	NULL	NULL	NULL	species specificity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to estimate the difference in interaction of human and rat factors with human APC and to assess the cause of the species specificity .
	manualset3
161703	6	411731	7	NULL	NULL	NULL	NULL	cause	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to estimate the difference in interaction of human and rat factors with human APC and to assess the cause of the species specificity .
	manualset3
160320	1	411732	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to examine the hypothesis that muscarinic receptor sensitivity is increased in depression .
	manualset3
160321	2	411732	7	NULL	NULL	0	NULL	hypothesis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to examine the hypothesis that muscarinic receptor sensitivity is increased in depression .
	manualset3
160322	3	411732	7	NULL	NULL	0	NULL	muscarinic receptor sensitivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to examine the hypothesis that muscarinic receptor sensitivity is increased in depression .
	manualset3
160323	4	411732	7	NULL	NULL	0	NULL	depression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to examine the hypothesis that muscarinic receptor sensitivity is increased in depression .
	manualset3
160324	1	411733	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to further examine the role of PKC system in growth regulation of gliomas in vitro by measurement of PKC activity over various phases of tumor growth and by assessing its potential role as a signal transduction system induced by serum mitogens and the known glioma mitogens epidermal growth factor and fibroblast growth factor .
	manualset3
160325	2	411733	7	NULL	NULL	0	NULL	PKC system	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to further examine the role of PKC system in growth regulation of gliomas in vitro by measurement of PKC activity over various phases of tumor growth and by assessing its potential role as a signal transduction system induced by serum mitogens and the known glioma mitogens epidermal growth factor and fibroblast growth factor .
	manualset3
160326	3	411733	7	NULL	NULL	0	NULL	growth regulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to further examine the role of PKC system in growth regulation of gliomas in vitro by measurement of PKC activity over various phases of tumor growth and by assessing its potential role as a signal transduction system induced by serum mitogens and the known glioma mitogens epidermal growth factor and fibroblast growth factor .
	manualset3
160327	4	411733	7	NULL	NULL	0	NULL	 gliomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to further examine the role of PKC system in growth regulation of gliomas in vitro by measurement of PKC activity over various phases of tumor growth and by assessing its potential role as a signal transduction system induced by serum mitogens and the known glioma mitogens epidermal growth factor and fibroblast growth factor .
	manualset3
160328	5	411733	7	NULL	NULL	0	NULL	PKC activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to further examine the role of PKC system in growth regulation of gliomas in vitro by measurement of PKC activity over various phases of tumor growth and by assessing its potential role as a signal transduction system induced by serum mitogens and the known glioma mitogens epidermal growth factor and fibroblast growth factor .
	manualset3
160329	6	411733	7	NULL	NULL	0	NULL	phases	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to further examine the role of PKC system in growth regulation of gliomas in vitro by measurement of PKC activity over various phases of tumor growth and by assessing its potential role as a signal transduction system induced by serum mitogens and the known glioma mitogens epidermal growth factor and fibroblast growth factor .
	manualset3
160330	7	411733	7	NULL	NULL	0	NULL	tumor growth 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to further examine the role of PKC system in growth regulation of gliomas in vitro by measurement of PKC activity over various phases of tumor growth and by assessing its potential role as a signal transduction system induced by serum mitogens and the known glioma mitogens epidermal growth factor and fibroblast growth factor .
	manualset3
160331	8	411733	7	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to further examine the role of PKC system in growth regulation of gliomas in vitro by measurement of PKC activity over various phases of tumor growth and by assessing its potential role as a signal transduction system induced by serum mitogens and the known glioma mitogens epidermal growth factor and fibroblast growth factor .
	manualset3
160332	9	411733	7	NULL	NULL	0	NULL	signal transduction system	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to further examine the role of PKC system in growth regulation of gliomas in vitro by measurement of PKC activity over various phases of tumor growth and by assessing its potential role as a signal transduction system induced by serum mitogens and the known glioma mitogens epidermal growth factor and fibroblast growth factor .
	manualset3
160333	10	411733	7	NULL	NULL	0	NULL	serum mitogens	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to further examine the role of PKC system in growth regulation of gliomas in vitro by measurement of PKC activity over various phases of tumor growth and by assessing its potential role as a signal transduction system induced by serum mitogens and the known glioma mitogens epidermal growth factor and fibroblast growth factor .
	manualset3
160334	11	411733	7	NULL	NULL	NULL	NULL	glioma mitogens	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to further examine the role of PKC system in growth regulation of gliomas in vitro by measurement of PKC activity over various phases of tumor growth and by assessing its potential role as a signal transduction system induced by serum mitogens and the known glioma mitogens epidermal growth factor and fibroblast growth factor .
	manualset3
160335	12	411733	7	NULL	NULL	0	NULL	epidermal growth factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to further examine the role of PKC system in growth regulation of gliomas in vitro by measurement of PKC activity over various phases of tumor growth and by assessing its potential role as a signal transduction system induced by serum mitogens and the known glioma mitogens epidermal growth factor and fibroblast growth factor .
	manualset3
160336	13	411733	7	NULL	NULL	0	NULL	fibroblast growth factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to further examine the role of PKC system in growth regulation of gliomas in vitro by measurement of PKC activity over various phases of tumor growth and by assessing its potential role as a signal transduction system induced by serum mitogens and the known glioma mitogens epidermal growth factor and fibroblast growth factor .
	manualset3
169201	14	411733	7	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to further examine the role of PKC system in growth regulation of gliomas in vitro by measurement of PKC activity over various phases of tumor growth and by assessing its potential role as a signal transduction system induced by serum mitogens and the known glioma mitogens epidermal growth factor and fibroblast growth factor .
	manualset3
169202	15	411733	7	NULL	NULL	0	NULL	 measurement	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study was undertaken to further examine the role of PKC system in growth regulation of gliomas in vitro by measurement of PKC activity over various phases of tumor growth and by assessing its potential role as a signal transduction system induced by serum mitogens and the known glioma mitogens epidermal growth factor and fibroblast growth factor .
	manualset3
160337	1	411734	7	NULL	NULL	0	NULL	surface graft polymerization method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present surface graft polymerization method , which is carried out under AP conditions , is particularly advantageous for polymer surface structuring via radical polymerization and can , in principle , be scaled to large surfaces .
	manualset3
160338	2	411734	7	NULL	NULL	0	NULL	AP conditions	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The present surface graft polymerization method , which is carried out under AP conditions , is particularly advantageous for polymer surface structuring via radical polymerization and can , in principle , be scaled to large surfaces .
	manualset3
160339	3	411734	7	NULL	NULL	NULL	NULL	polymer surface structuring	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present surface graft polymerization method , which is carried out under AP conditions , is particularly advantageous for polymer surface structuring via radical polymerization and can , in principle , be scaled to large surfaces .
	manualset3
160340	4	411734	7	NULL	NULL	0	NULL	radical polymerization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present surface graft polymerization method , which is carried out under AP conditions , is particularly advantageous for polymer surface structuring via radical polymerization and can , in principle , be scaled to large surfaces .
	manualset3
161704	5	411734	7	NULL	NULL	0	NULL	large surfaces	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present surface graft polymerization method , which is carried out under AP conditions , is particularly advantageous for polymer surface structuring via radical polymerization and can , in principle , be scaled to large surfaces .
	manualset3
160341	1	411735	7	NULL	NULL	0	NULL	system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The present system uses a set of arithmetic logic rules which allows comprehensive evaluation of laboratory data as well as bringing into focus fluctuating and borderline situations and inconclusive data .
	manualset3
160342	2	411735	7	NULL	NULL	0	NULL	set	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The present system uses a set of arithmetic logic rules which allows comprehensive evaluation of laboratory data as well as bringing into focus fluctuating and borderline situations and inconclusive data .
	manualset3
160343	3	411735	7	NULL	NULL	0	NULL	arithmetic logic rules	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The present system uses a set of arithmetic logic rules which allows comprehensive evaluation of laboratory data as well as bringing into focus fluctuating and borderline situations and inconclusive data .
	manualset3
160344	4	411735	7	NULL	NULL	0	NULL	 evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present system uses a set of arithmetic logic rules which allows comprehensive evaluation of laboratory data as well as bringing into focus fluctuating and borderline situations and inconclusive data .
	manualset3
160345	5	411735	7	NULL	NULL	0	NULL	laboratory data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The present system uses a set of arithmetic logic rules which allows comprehensive evaluation of laboratory data as well as bringing into focus fluctuating and borderline situations and inconclusive data .
	manualset3
160346	6	411735	7	NULL	NULL	0	NULL	focus fluctuating situations	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present system uses a set of arithmetic logic rules which allows comprehensive evaluation of laboratory data as well as bringing into focus fluctuating and borderline situations and inconclusive data .
	manualset3
160347	7	411735	7	NULL	NULL	0	NULL	borderline situations	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present system uses a set of arithmetic logic rules which allows comprehensive evaluation of laboratory data as well as bringing into focus fluctuating and borderline situations and inconclusive data .
	manualset3
160348	8	411735	7	NULL	NULL	0	NULL	inconclusive data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The present system uses a set of arithmetic logic rules which allows comprehensive evaluation of laboratory data as well as bringing into focus fluctuating and borderline situations and inconclusive data .
	manualset3
160349	1	411736	7	NULL	NULL	NULL	NULL	AREAS COVERED	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	AREAS COVERED : In recent years , small-molecule inhibitors of Hh signaling have been synthesized for cancer treatment .
	manualset3
160350	2	411736	7	NULL	NULL	0	NULL	years	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	AREAS COVERED : In recent years , small-molecule inhibitors of Hh signaling have been synthesized for cancer treatment .
	manualset3
160351	3	411736	7	NULL	NULL	0	NULL	small-molecule inhibitors	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	AREAS COVERED : In recent years , small-molecule inhibitors of Hh signaling have been synthesized for cancer treatment .
	manualset3
160352	4	411736	7	NULL	NULL	0	NULL	Hh signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	AREAS COVERED : In recent years , small-molecule inhibitors of Hh signaling have been synthesized for cancer treatment .
	manualset3
160353	5	411736	7	NULL	NULL	NULL	NULL	cancer treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	AREAS COVERED : In recent years , small-molecule inhibitors of Hh signaling have been synthesized for cancer treatment .
	manualset3
160354	1	411737	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The present treatment outcome study was designed to determine the extent to which Interactive-Behavioral Training ( IBT ) -- a group psychotherapy model that actively combines cognitive-behavioral and group process techniques -- can provide significant gains for people who suffer from chronic and debilitating social impairment and negative symptoms .
	manualset3
160355	2	411737	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present treatment outcome study was designed to determine the extent to which Interactive-Behavioral Training ( IBT ) -- a group psychotherapy model that actively combines cognitive-behavioral and group process techniques -- can provide significant gains for people who suffer from chronic and debilitating social impairment and negative symptoms .
	manualset3
160356	3	411737	7	NULL	NULL	0	NULL	extent	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present treatment outcome study was designed to determine the extent to which Interactive-Behavioral Training ( IBT ) -- a group psychotherapy model that actively combines cognitive-behavioral and group process techniques -- can provide significant gains for people who suffer from chronic and debilitating social impairment and negative symptoms .
	manualset3
160357	4	411737	7	NULL	NULL	0	NULL	Interactive-Behavioral Training ( IBT )	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The present treatment outcome study was designed to determine the extent to which Interactive-Behavioral Training ( IBT ) -- a group psychotherapy model that actively combines cognitive-behavioral and group process techniques -- can provide significant gains for people who suffer from chronic and debilitating social impairment and negative symptoms .
	manualset3
160358	5	411737	7	NULL	NULL	0	NULL	group psychotherapy model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The present treatment outcome study was designed to determine the extent to which Interactive-Behavioral Training ( IBT ) -- a group psychotherapy model that actively combines cognitive-behavioral and group process techniques -- can provide significant gains for people who suffer from chronic and debilitating social impairment and negative symptoms .
	manualset3
160359	6	411737	7	NULL	NULL	NULL	NULL	cognitive-behavioral techniques	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present treatment outcome study was designed to determine the extent to which Interactive-Behavioral Training ( IBT ) -- a group psychotherapy model that actively combines cognitive-behavioral and group process techniques -- can provide significant gains for people who suffer from chronic and debilitating social impairment and negative symptoms .
	manualset3
160360	7	411737	7	NULL	NULL	NULL	NULL	group process techniques	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present treatment outcome study was designed to determine the extent to which Interactive-Behavioral Training ( IBT ) -- a group psychotherapy model that actively combines cognitive-behavioral and group process techniques -- can provide significant gains for people who suffer from chronic and debilitating social impairment and negative symptoms .
	manualset3
160361	8	411737	7	NULL	NULL	0	NULL	people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The present treatment outcome study was designed to determine the extent to which Interactive-Behavioral Training ( IBT ) -- a group psychotherapy model that actively combines cognitive-behavioral and group process techniques -- can provide significant gains for people who suffer from chronic and debilitating social impairment and negative symptoms .
	manualset3
160362	9	411737	7	NULL	NULL	0	NULL	chronic and debilitating social impairment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present treatment outcome study was designed to determine the extent to which Interactive-Behavioral Training ( IBT ) -- a group psychotherapy model that actively combines cognitive-behavioral and group process techniques -- can provide significant gains for people who suffer from chronic and debilitating social impairment and negative symptoms .
	manualset3
160363	10	411737	7	NULL	NULL	0	NULL	negative symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present treatment outcome study was designed to determine the extent to which Interactive-Behavioral Training ( IBT ) -- a group psychotherapy model that actively combines cognitive-behavioral and group process techniques -- can provide significant gains for people who suffer from chronic and debilitating social impairment and negative symptoms .
	manualset3
160364	1	411738	7	NULL	NULL	0	NULL	work	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present work provides evidence that resveratrol reduces the formation of prostaglandins in neuroblastoma cells by reducing the enzymatic activity of inducible enzymes , such as COX-2 , and not the transcription of the PG synthases , as demonstrated elsewhere .
	manualset3
160365	2	411738	7	NULL	NULL	0	NULL	evidence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present work provides evidence that resveratrol reduces the formation of prostaglandins in neuroblastoma cells by reducing the enzymatic activity of inducible enzymes , such as COX-2 , and not the transcription of the PG synthases , as demonstrated elsewhere .
	manualset3
160366	3	411738	7	NULL	NULL	0	NULL	resveratrol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The present work provides evidence that resveratrol reduces the formation of prostaglandins in neuroblastoma cells by reducing the enzymatic activity of inducible enzymes , such as COX-2 , and not the transcription of the PG synthases , as demonstrated elsewhere .
	manualset3
160367	4	411738	7	NULL	NULL	0	NULL	formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present work provides evidence that resveratrol reduces the formation of prostaglandins in neuroblastoma cells by reducing the enzymatic activity of inducible enzymes , such as COX-2 , and not the transcription of the PG synthases , as demonstrated elsewhere .
	manualset3
160368	5	411738	7	NULL	NULL	0	NULL	prostaglandins	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present work provides evidence that resveratrol reduces the formation of prostaglandins in neuroblastoma cells by reducing the enzymatic activity of inducible enzymes , such as COX-2 , and not the transcription of the PG synthases , as demonstrated elsewhere .
	manualset3
160369	6	411738	7	NULL	NULL	0	NULL	neuroblastoma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The present work provides evidence that resveratrol reduces the formation of prostaglandins in neuroblastoma cells by reducing the enzymatic activity of inducible enzymes , such as COX-2 , and not the transcription of the PG synthases , as demonstrated elsewhere .
	manualset3
160370	7	411738	7	NULL	NULL	0	NULL	enzymatic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present work provides evidence that resveratrol reduces the formation of prostaglandins in neuroblastoma cells by reducing the enzymatic activity of inducible enzymes , such as COX-2 , and not the transcription of the PG synthases , as demonstrated elsewhere .
	manualset3
160371	8	411738	7	NULL	NULL	0	NULL	inducible enzymes	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present work provides evidence that resveratrol reduces the formation of prostaglandins in neuroblastoma cells by reducing the enzymatic activity of inducible enzymes , such as COX-2 , and not the transcription of the PG synthases , as demonstrated elsewhere .
	manualset3
160372	9	411738	7	NULL	NULL	0	NULL	COX-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present work provides evidence that resveratrol reduces the formation of prostaglandins in neuroblastoma cells by reducing the enzymatic activity of inducible enzymes , such as COX-2 , and not the transcription of the PG synthases , as demonstrated elsewhere .
	manualset3
160373	10	411738	7	NULL	NULL	0	NULL	transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present work provides evidence that resveratrol reduces the formation of prostaglandins in neuroblastoma cells by reducing the enzymatic activity of inducible enzymes , such as COX-2 , and not the transcription of the PG synthases , as demonstrated elsewhere .
	manualset3
160374	11	411738	7	NULL	NULL	0	NULL	PG synthases	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present work provides evidence that resveratrol reduces the formation of prostaglandins in neuroblastoma cells by reducing the enzymatic activity of inducible enzymes , such as COX-2 , and not the transcription of the PG synthases , as demonstrated elsewhere .
	manualset3
160376	1	411739	7	NULL	NULL	0	NULL	presentation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presentation , aetiology and treatment are described and the importance of including it in the differential diagnosis is discussed .
	manualset3
160377	2	411739	7	NULL	NULL	0	NULL	 aetiology	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presentation , aetiology and treatment are described and the importance of including it in the differential diagnosis is discussed .
	manualset3
160378	3	411739	7	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The presentation , aetiology and treatment are described and the importance of including it in the differential diagnosis is discussed .
	manualset3
160379	4	411739	7	NULL	NULL	0	NULL	differential diagnosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The presentation , aetiology and treatment are described and the importance of including it in the differential diagnosis is discussed .
	manualset3
160380	1	411740	7	NULL	NULL	0	NULL	presentation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presentation is usually that of SIADH , but the underlying mechanism leading to the syndrome is poorly understood .
	manualset3
160381	2	411740	7	NULL	NULL	0	NULL	SIADH	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The presentation is usually that of SIADH , but the underlying mechanism leading to the syndrome is poorly understood .
	manualset3
160382	3	411740	7	NULL	NULL	0	NULL	mechanism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presentation is usually that of SIADH , but the underlying mechanism leading to the syndrome is poorly understood .
	manualset3
160383	4	411740	7	NULL	NULL	0	NULL	syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The presentation is usually that of SIADH , but the underlying mechanism leading to the syndrome is poorly understood .
	manualset3
160384	1	411741	7	NULL	NULL	0	NULL	presentation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The presentation is usually with abdominal pain .
	manualset3
160385	2	411741	7	NULL	NULL	0	NULL	abdominal pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The presentation is usually with abdominal pain .
	manualset3
160386	1	411742	7	NULL	NULL	0	NULL	algorithm	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The presented algorithm is semiautomated giving objective results based on predefined criteria with the option of user intervention .
	manualset3
160387	2	411742	7	NULL	NULL	0	NULL	objective results	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presented algorithm is semiautomated giving objective results based on predefined criteria with the option of user intervention .
	manualset3
160388	3	411742	7	NULL	NULL	0	NULL	criteria	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presented algorithm is semiautomated giving objective results based on predefined criteria with the option of user intervention .
	manualset3
160389	4	411742	7	NULL	NULL	0	NULL	user intervention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presented algorithm is semiautomated giving objective results based on predefined criteria with the option of user intervention .
	manualset3
169203	5	411742	7	NULL	NULL	0	NULL	option	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presented algorithm is semiautomated giving objective results based on predefined criteria with the option of user intervention .
	manualset3
160390	1	411743	7	NULL	NULL	NULL	NULL	pressure	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The pressure remained at normal value ( 15.7 mmHg ) .
	manualset3
160391	2	411743	7	NULL	NULL	0	NULL	normal value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The pressure remained at normal value ( 15.7 mmHg ) .
	manualset3
160392	3	411743	7	NULL	NULL	0	NULL	15.7 mmHg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The pressure remained at normal value ( 15.7 mmHg ) .
	manualset3
160393	1	411744	7	NULL	NULL	0	NULL	pressure variations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The pressure variations are proposed to represent peristaltic activity with the ability of expelling the last drops of urine after micturition and posing a mechanical barrier to ascending microorganisms .
	manualset3
160395	2	411744	7	NULL	NULL	0	NULL	peristaltic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The pressure variations are proposed to represent peristaltic activity with the ability of expelling the last drops of urine after micturition and posing a mechanical barrier to ascending microorganisms .
	manualset3
160396	3	411744	7	NULL	NULL	NULL	NULL	expelling 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The pressure variations are proposed to represent peristaltic activity with the ability of expelling the last drops of urine after micturition and posing a mechanical barrier to ascending microorganisms .
	manualset3
160397	4	411744	7	NULL	NULL	0	NULL	micturition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The pressure variations are proposed to represent peristaltic activity with the ability of expelling the last drops of urine after micturition and posing a mechanical barrier to ascending microorganisms .
	manualset3
160398	5	411744	7	NULL	NULL	NULL	NULL	mechanical barrier	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The pressure variations are proposed to represent peristaltic activity with the ability of expelling the last drops of urine after micturition and posing a mechanical barrier to ascending microorganisms .
	manualset3
160399	6	411744	7	NULL	NULL	0	NULL	microorganisms 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The pressure variations are proposed to represent peristaltic activity with the ability of expelling the last drops of urine after micturition and posing a mechanical barrier to ascending microorganisms .
	manualset3
160400	7	411744	7	NULL	NULL	NULL	NULL	 last drops of urine	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The pressure variations are proposed to represent peristaltic activity with the ability of expelling the last drops of urine after micturition and posing a mechanical barrier to ascending microorganisms .
	manualset3
160401	8	411744	7	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The pressure variations are proposed to represent peristaltic activity with the ability of expelling the last drops of urine after micturition and posing a mechanical barrier to ascending microorganisms .
	manualset3
160402	1	411745	7	NULL	NULL	0	NULL	pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The pressure will exert an effect upon the optic disc which either directly on the nerve fibers or indirectly via the vascular system will result in a characteristic optic atrophy .
	manualset3
160403	2	411745	7	NULL	NULL	0	NULL	optic disc	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The pressure will exert an effect upon the optic disc which either directly on the nerve fibers or indirectly via the vascular system will result in a characteristic optic atrophy .
	manualset3
160404	3	411745	7	NULL	NULL	0	NULL	nerve fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The pressure will exert an effect upon the optic disc which either directly on the nerve fibers or indirectly via the vascular system will result in a characteristic optic atrophy .
	manualset3
160405	4	411745	7	NULL	NULL	0	NULL	vascular system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The pressure will exert an effect upon the optic disc which either directly on the nerve fibers or indirectly via the vascular system will result in a characteristic optic atrophy .
	manualset3
160406	5	411745	7	NULL	NULL	0	NULL	optic atrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The pressure will exert an effect upon the optic disc which either directly on the nerve fibers or indirectly via the vascular system will result in a characteristic optic atrophy .
	manualset3
160407	6	411745	7	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The pressure will exert an effect upon the optic disc which either directly on the nerve fibers or indirectly via the vascular system will result in a characteristic optic atrophy .
	manualset3
160408	1	411746	7	NULL	NULL	0	NULL	presynaptic action	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The presynaptic action of GABA and the neural transmitter was depressed by picrotoxin .
	manualset3
160409	2	411746	7	NULL	NULL	0	NULL	GABA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The presynaptic action of GABA and the neural transmitter was depressed by picrotoxin .
	manualset3
160410	3	411746	7	NULL	NULL	0	NULL	neural transmitter	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The presynaptic action of GABA and the neural transmitter was depressed by picrotoxin .
	manualset3
160411	4	411746	7	NULL	NULL	0	NULL	picrotoxin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The presynaptic action of GABA and the neural transmitter was depressed by picrotoxin .
	manualset3
160412	1	411747	7	NULL	NULL	0	NULL	AREAS COVERED	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	AREAS COVERED : NK cells play important roles in viral infections , autoimmunity , pregnancy , cancer and bone marrow transplantation .
	manualset3
160413	2	411747	7	NULL	NULL	0	NULL	NK cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	AREAS COVERED : NK cells play important roles in viral infections , autoimmunity , pregnancy , cancer and bone marrow transplantation .
	manualset3
160414	3	411747	7	NULL	NULL	0	NULL	roles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	AREAS COVERED : NK cells play important roles in viral infections , autoimmunity , pregnancy , cancer and bone marrow transplantation .
	manualset3
160415	4	411747	7	NULL	NULL	0	NULL	viral infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	AREAS COVERED : NK cells play important roles in viral infections , autoimmunity , pregnancy , cancer and bone marrow transplantation .
	manualset3
160416	5	411747	7	NULL	NULL	0	NULL	autoimmunity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	AREAS COVERED : NK cells play important roles in viral infections , autoimmunity , pregnancy , cancer and bone marrow transplantation .
	manualset3
160417	6	411747	7	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	AREAS COVERED : NK cells play important roles in viral infections , autoimmunity , pregnancy , cancer and bone marrow transplantation .
	manualset3
160418	7	411747	7	NULL	NULL	NULL	NULL	 cancer	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	AREAS COVERED : NK cells play important roles in viral infections , autoimmunity , pregnancy , cancer and bone marrow transplantation .
	manualset3
160419	8	411747	7	NULL	NULL	0	NULL	bone marrow transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	AREAS COVERED : NK cells play important roles in viral infections , autoimmunity , pregnancy , cancer and bone marrow transplantation .
	manualset3
160420	1	411748	7	NULL	NULL	0	NULL	pretreatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The pretreatment of lymphocytes with H89 , a cell-permeable PKA inhibitor , prevents the induction of anergy .
	manualset3
160421	2	411748	7	NULL	NULL	0	NULL	 lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The pretreatment of lymphocytes with H89 , a cell-permeable PKA inhibitor , prevents the induction of anergy .
	manualset3
160422	3	411748	7	NULL	NULL	0	NULL	H89	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The pretreatment of lymphocytes with H89 , a cell-permeable PKA inhibitor , prevents the induction of anergy .
	manualset3
160423	4	411748	7	NULL	NULL	0	NULL	cell-permeable PKA inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The pretreatment of lymphocytes with H89 , a cell-permeable PKA inhibitor , prevents the induction of anergy .
	manualset3
160424	5	411748	7	NULL	NULL	NULL	NULL	induction 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The pretreatment of lymphocytes with H89 , a cell-permeable PKA inhibitor , prevents the induction of anergy .
	manualset3
160425	6	411748	7	NULL	NULL	0	NULL	anergy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The pretreatment of lymphocytes with H89 , a cell-permeable PKA inhibitor , prevents the induction of anergy .
	manualset3
160426	1	411749	7	NULL	NULL	0	NULL	prevalence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence ( number positive/number tested in production type ) of Cd was different between the groups ( P & lt ; or = 0.001 ) , and was highest among suckling piglets at 50.0 % ( 61/122 ) , followed by 23.8 % ( 34/143 ) for lactating sows and effluent from the farrowing barn , 8.4 % ( 10/119 ) for nursery , 6.5 % ( 4/62 ) for pork products , 3.9 % ( 15/382 ) for grower-finisher , and 3.9 % ( 7/180 ) for breeding boars and sows .
	manualset3
160427	2	411749	7	NULL	NULL	0	NULL	 number positive/number tested in production type	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence ( number positive/number tested in production type ) of Cd was different between the groups ( P & lt ; or = 0.001 ) , and was highest among suckling piglets at 50.0 % ( 61/122 ) , followed by 23.8 % ( 34/143 ) for lactating sows and effluent from the farrowing barn , 8.4 % ( 10/119 ) for nursery , 6.5 % ( 4/62 ) for pork products , 3.9 % ( 15/382 ) for grower-finisher , and 3.9 % ( 7/180 ) for breeding boars and sows .
	manualset3
160428	3	411749	7	NULL	NULL	0	NULL	Cd	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence ( number positive/number tested in production type ) of Cd was different between the groups ( P & lt ; or = 0.001 ) , and was highest among suckling piglets at 50.0 % ( 61/122 ) , followed by 23.8 % ( 34/143 ) for lactating sows and effluent from the farrowing barn , 8.4 % ( 10/119 ) for nursery , 6.5 % ( 4/62 ) for pork products , 3.9 % ( 15/382 ) for grower-finisher , and 3.9 % ( 7/180 ) for breeding boars and sows .
	manualset3
160429	4	411749	7	NULL	NULL	NULL	NULL	 groups	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The prevalence ( number positive/number tested in production type ) of Cd was different between the groups ( P & lt ; or = 0.001 ) , and was highest among suckling piglets at 50.0 % ( 61/122 ) , followed by 23.8 % ( 34/143 ) for lactating sows and effluent from the farrowing barn , 8.4 % ( 10/119 ) for nursery , 6.5 % ( 4/62 ) for pork products , 3.9 % ( 15/382 ) for grower-finisher , and 3.9 % ( 7/180 ) for breeding boars and sows .
	manualset3
160430	5	411749	7	NULL	NULL	0	NULL	P & lt ; or = 0.001 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence ( number positive/number tested in production type ) of Cd was different between the groups ( P & lt ; or = 0.001 ) , and was highest among suckling piglets at 50.0 % ( 61/122 ) , followed by 23.8 % ( 34/143 ) for lactating sows and effluent from the farrowing barn , 8.4 % ( 10/119 ) for nursery , 6.5 % ( 4/62 ) for pork products , 3.9 % ( 15/382 ) for grower-finisher , and 3.9 % ( 7/180 ) for breeding boars and sows .
	manualset3
160431	6	411749	7	NULL	NULL	0	NULL	suckling piglets	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence ( number positive/number tested in production type ) of Cd was different between the groups ( P & lt ; or = 0.001 ) , and was highest among suckling piglets at 50.0 % ( 61/122 ) , followed by 23.8 % ( 34/143 ) for lactating sows and effluent from the farrowing barn , 8.4 % ( 10/119 ) for nursery , 6.5 % ( 4/62 ) for pork products , 3.9 % ( 15/382 ) for grower-finisher , and 3.9 % ( 7/180 ) for breeding boars and sows .
	manualset3
160432	7	411749	7	NULL	NULL	0	NULL	50.0 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence ( number positive/number tested in production type ) of Cd was different between the groups ( P & lt ; or = 0.001 ) , and was highest among suckling piglets at 50.0 % ( 61/122 ) , followed by 23.8 % ( 34/143 ) for lactating sows and effluent from the farrowing barn , 8.4 % ( 10/119 ) for nursery , 6.5 % ( 4/62 ) for pork products , 3.9 % ( 15/382 ) for grower-finisher , and 3.9 % ( 7/180 ) for breeding boars and sows .
	manualset3
160433	8	411749	7	NULL	NULL	0	NULL	61/122 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence ( number positive/number tested in production type ) of Cd was different between the groups ( P & lt ; or = 0.001 ) , and was highest among suckling piglets at 50.0 % ( 61/122 ) , followed by 23.8 % ( 34/143 ) for lactating sows and effluent from the farrowing barn , 8.4 % ( 10/119 ) for nursery , 6.5 % ( 4/62 ) for pork products , 3.9 % ( 15/382 ) for grower-finisher , and 3.9 % ( 7/180 ) for breeding boars and sows .
	manualset3
160434	9	411749	7	NULL	NULL	0	NULL	23.8 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence ( number positive/number tested in production type ) of Cd was different between the groups ( P & lt ; or = 0.001 ) , and was highest among suckling piglets at 50.0 % ( 61/122 ) , followed by 23.8 % ( 34/143 ) for lactating sows and effluent from the farrowing barn , 8.4 % ( 10/119 ) for nursery , 6.5 % ( 4/62 ) for pork products , 3.9 % ( 15/382 ) for grower-finisher , and 3.9 % ( 7/180 ) for breeding boars and sows .
	manualset3
160435	10	411749	7	NULL	NULL	0	NULL	 34/143	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence ( number positive/number tested in production type ) of Cd was different between the groups ( P & lt ; or = 0.001 ) , and was highest among suckling piglets at 50.0 % ( 61/122 ) , followed by 23.8 % ( 34/143 ) for lactating sows and effluent from the farrowing barn , 8.4 % ( 10/119 ) for nursery , 6.5 % ( 4/62 ) for pork products , 3.9 % ( 15/382 ) for grower-finisher , and 3.9 % ( 7/180 ) for breeding boars and sows .
	manualset3
160436	11	411749	7	NULL	NULL	0	NULL	lactating sows 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence ( number positive/number tested in production type ) of Cd was different between the groups ( P & lt ; or = 0.001 ) , and was highest among suckling piglets at 50.0 % ( 61/122 ) , followed by 23.8 % ( 34/143 ) for lactating sows and effluent from the farrowing barn , 8.4 % ( 10/119 ) for nursery , 6.5 % ( 4/62 ) for pork products , 3.9 % ( 15/382 ) for grower-finisher , and 3.9 % ( 7/180 ) for breeding boars and sows .
	manualset3
160437	12	411749	7	NULL	NULL	0	NULL	 effluent 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence ( number positive/number tested in production type ) of Cd was different between the groups ( P & lt ; or = 0.001 ) , and was highest among suckling piglets at 50.0 % ( 61/122 ) , followed by 23.8 % ( 34/143 ) for lactating sows and effluent from the farrowing barn , 8.4 % ( 10/119 ) for nursery , 6.5 % ( 4/62 ) for pork products , 3.9 % ( 15/382 ) for grower-finisher , and 3.9 % ( 7/180 ) for breeding boars and sows .
	manualset3
160438	13	411749	7	NULL	NULL	0	NULL	farrowing barn	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence ( number positive/number tested in production type ) of Cd was different between the groups ( P & lt ; or = 0.001 ) , and was highest among suckling piglets at 50.0 % ( 61/122 ) , followed by 23.8 % ( 34/143 ) for lactating sows and effluent from the farrowing barn , 8.4 % ( 10/119 ) for nursery , 6.5 % ( 4/62 ) for pork products , 3.9 % ( 15/382 ) for grower-finisher , and 3.9 % ( 7/180 ) for breeding boars and sows .
	manualset3
160439	14	411749	7	NULL	NULL	0	NULL	8.4 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence ( number positive/number tested in production type ) of Cd was different between the groups ( P & lt ; or = 0.001 ) , and was highest among suckling piglets at 50.0 % ( 61/122 ) , followed by 23.8 % ( 34/143 ) for lactating sows and effluent from the farrowing barn , 8.4 % ( 10/119 ) for nursery , 6.5 % ( 4/62 ) for pork products , 3.9 % ( 15/382 ) for grower-finisher , and 3.9 % ( 7/180 ) for breeding boars and sows .
	manualset3
160440	15	411749	7	NULL	NULL	0	NULL	10/119	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence ( number positive/number tested in production type ) of Cd was different between the groups ( P & lt ; or = 0.001 ) , and was highest among suckling piglets at 50.0 % ( 61/122 ) , followed by 23.8 % ( 34/143 ) for lactating sows and effluent from the farrowing barn , 8.4 % ( 10/119 ) for nursery , 6.5 % ( 4/62 ) for pork products , 3.9 % ( 15/382 ) for grower-finisher , and 3.9 % ( 7/180 ) for breeding boars and sows .
	manualset3
160441	16	411749	7	NULL	NULL	0	NULL	nursery	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence ( number positive/number tested in production type ) of Cd was different between the groups ( P & lt ; or = 0.001 ) , and was highest among suckling piglets at 50.0 % ( 61/122 ) , followed by 23.8 % ( 34/143 ) for lactating sows and effluent from the farrowing barn , 8.4 % ( 10/119 ) for nursery , 6.5 % ( 4/62 ) for pork products , 3.9 % ( 15/382 ) for grower-finisher , and 3.9 % ( 7/180 ) for breeding boars and sows .
	manualset3
160442	17	411749	7	NULL	NULL	0	NULL	 6.5 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence ( number positive/number tested in production type ) of Cd was different between the groups ( P & lt ; or = 0.001 ) , and was highest among suckling piglets at 50.0 % ( 61/122 ) , followed by 23.8 % ( 34/143 ) for lactating sows and effluent from the farrowing barn , 8.4 % ( 10/119 ) for nursery , 6.5 % ( 4/62 ) for pork products , 3.9 % ( 15/382 ) for grower-finisher , and 3.9 % ( 7/180 ) for breeding boars and sows .
	manualset3
160443	18	411749	7	NULL	NULL	0	NULL	4/62	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence ( number positive/number tested in production type ) of Cd was different between the groups ( P & lt ; or = 0.001 ) , and was highest among suckling piglets at 50.0 % ( 61/122 ) , followed by 23.8 % ( 34/143 ) for lactating sows and effluent from the farrowing barn , 8.4 % ( 10/119 ) for nursery , 6.5 % ( 4/62 ) for pork products , 3.9 % ( 15/382 ) for grower-finisher , and 3.9 % ( 7/180 ) for breeding boars and sows .
	manualset3
160444	19	411749	7	NULL	NULL	0	NULL	pork products	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence ( number positive/number tested in production type ) of Cd was different between the groups ( P & lt ; or = 0.001 ) , and was highest among suckling piglets at 50.0 % ( 61/122 ) , followed by 23.8 % ( 34/143 ) for lactating sows and effluent from the farrowing barn , 8.4 % ( 10/119 ) for nursery , 6.5 % ( 4/62 ) for pork products , 3.9 % ( 15/382 ) for grower-finisher , and 3.9 % ( 7/180 ) for breeding boars and sows .
	manualset3
160445	20	411749	7	NULL	NULL	0	NULL	 3.9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence ( number positive/number tested in production type ) of Cd was different between the groups ( P & lt ; or = 0.001 ) , and was highest among suckling piglets at 50.0 % ( 61/122 ) , followed by 23.8 % ( 34/143 ) for lactating sows and effluent from the farrowing barn , 8.4 % ( 10/119 ) for nursery , 6.5 % ( 4/62 ) for pork products , 3.9 % ( 15/382 ) for grower-finisher , and 3.9 % ( 7/180 ) for breeding boars and sows .
	manualset3
160446	21	411749	7	NULL	NULL	0	NULL	15/382	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence ( number positive/number tested in production type ) of Cd was different between the groups ( P & lt ; or = 0.001 ) , and was highest among suckling piglets at 50.0 % ( 61/122 ) , followed by 23.8 % ( 34/143 ) for lactating sows and effluent from the farrowing barn , 8.4 % ( 10/119 ) for nursery , 6.5 % ( 4/62 ) for pork products , 3.9 % ( 15/382 ) for grower-finisher , and 3.9 % ( 7/180 ) for breeding boars and sows .
	manualset3
160447	22	411749	7	NULL	NULL	0	NULL	grower-finisher	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence ( number positive/number tested in production type ) of Cd was different between the groups ( P & lt ; or = 0.001 ) , and was highest among suckling piglets at 50.0 % ( 61/122 ) , followed by 23.8 % ( 34/143 ) for lactating sows and effluent from the farrowing barn , 8.4 % ( 10/119 ) for nursery , 6.5 % ( 4/62 ) for pork products , 3.9 % ( 15/382 ) for grower-finisher , and 3.9 % ( 7/180 ) for breeding boars and sows .
	manualset3
160448	23	411749	7	NULL	NULL	0	NULL	 breeding boars 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence ( number positive/number tested in production type ) of Cd was different between the groups ( P & lt ; or = 0.001 ) , and was highest among suckling piglets at 50.0 % ( 61/122 ) , followed by 23.8 % ( 34/143 ) for lactating sows and effluent from the farrowing barn , 8.4 % ( 10/119 ) for nursery , 6.5 % ( 4/62 ) for pork products , 3.9 % ( 15/382 ) for grower-finisher , and 3.9 % ( 7/180 ) for breeding boars and sows .
	manualset3
160449	24	411749	7	NULL	NULL	0	NULL	 breeding sows	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence ( number positive/number tested in production type ) of Cd was different between the groups ( P & lt ; or = 0.001 ) , and was highest among suckling piglets at 50.0 % ( 61/122 ) , followed by 23.8 % ( 34/143 ) for lactating sows and effluent from the farrowing barn , 8.4 % ( 10/119 ) for nursery , 6.5 % ( 4/62 ) for pork products , 3.9 % ( 15/382 ) for grower-finisher , and 3.9 % ( 7/180 ) for breeding boars and sows .
	manualset3
161705	25	411749	7	NULL	NULL	0	NULL	 3.9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence ( number positive/number tested in production type ) of Cd was different between the groups ( P & lt ; or = 0.001 ) , and was highest among suckling piglets at 50.0 % ( 61/122 ) , followed by 23.8 % ( 34/143 ) for lactating sows and effluent from the farrowing barn , 8.4 % ( 10/119 ) for nursery , 6.5 % ( 4/62 ) for pork products , 3.9 % ( 15/382 ) for grower-finisher , and 3.9 % ( 7/180 ) for breeding boars and sows .
	manualset3
161706	26	411749	7	NULL	NULL	0	NULL	7/180	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence ( number positive/number tested in production type ) of Cd was different between the groups ( P & lt ; or = 0.001 ) , and was highest among suckling piglets at 50.0 % ( 61/122 ) , followed by 23.8 % ( 34/143 ) for lactating sows and effluent from the farrowing barn , 8.4 % ( 10/119 ) for nursery , 6.5 % ( 4/62 ) for pork products , 3.9 % ( 15/382 ) for grower-finisher , and 3.9 % ( 7/180 ) for breeding boars and sows .
	manualset3
160450	1	411750	7	NULL	NULL	NULL	NULL	prevalence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The prevalence of Helicobacter pylori infection is variable in different countries .
	manualset3
160451	2	411750	7	NULL	NULL	0	NULL	Helicobacter pylori infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of Helicobacter pylori infection is variable in different countries .
	manualset3
160453	4	411750	7	NULL	NULL	0	NULL	countries	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of Helicobacter pylori infection is variable in different countries .
	manualset3
160454	1	411751	7	NULL	NULL	0	NULL	prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of antibodies to HTLV-I in the Slovenian population might be somewhere between one in 10 , 000 ( 0.01 % ) and one in 15 , 000 ( 0.0066 % ) , which is similar or even higher to prevalence rates in other European countries .
	manualset3
160455	2	411751	7	NULL	NULL	0	NULL	antibodies 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of antibodies to HTLV-I in the Slovenian population might be somewhere between one in 10 , 000 ( 0.01 % ) and one in 15 , 000 ( 0.0066 % ) , which is similar or even higher to prevalence rates in other European countries .
	manualset3
160456	3	411751	7	NULL	NULL	0	NULL	HTLV-I	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of antibodies to HTLV-I in the Slovenian population might be somewhere between one in 10 , 000 ( 0.01 % ) and one in 15 , 000 ( 0.0066 % ) , which is similar or even higher to prevalence rates in other European countries .
	manualset3
160457	4	411751	7	NULL	NULL	0	NULL	Slovenian population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of antibodies to HTLV-I in the Slovenian population might be somewhere between one in 10 , 000 ( 0.01 % ) and one in 15 , 000 ( 0.0066 % ) , which is similar or even higher to prevalence rates in other European countries .
	manualset3
160458	5	411751	7	NULL	NULL	0	NULL	one in 10 , 000	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of antibodies to HTLV-I in the Slovenian population might be somewhere between one in 10 , 000 ( 0.01 % ) and one in 15 , 000 ( 0.0066 % ) , which is similar or even higher to prevalence rates in other European countries .
	manualset3
160459	6	411751	7	NULL	NULL	0	NULL	 0.01 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of antibodies to HTLV-I in the Slovenian population might be somewhere between one in 10 , 000 ( 0.01 % ) and one in 15 , 000 ( 0.0066 % ) , which is similar or even higher to prevalence rates in other European countries .
	manualset3
160460	7	411751	7	NULL	NULL	0	NULL	one in 15 , 000	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of antibodies to HTLV-I in the Slovenian population might be somewhere between one in 10 , 000 ( 0.01 % ) and one in 15 , 000 ( 0.0066 % ) , which is similar or even higher to prevalence rates in other European countries .
	manualset3
160461	8	411751	7	NULL	NULL	0	NULL	0.0066 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of antibodies to HTLV-I in the Slovenian population might be somewhere between one in 10 , 000 ( 0.01 % ) and one in 15 , 000 ( 0.0066 % ) , which is similar or even higher to prevalence rates in other European countries .
	manualset3
160463	9	411751	7	NULL	NULL	0	NULL	European countries	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of antibodies to HTLV-I in the Slovenian population might be somewhere between one in 10 , 000 ( 0.01 % ) and one in 15 , 000 ( 0.0066 % ) , which is similar or even higher to prevalence rates in other European countries .
	manualset3
169223	10	411751	7	NULL	NULL	0	NULL	prevalence rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of antibodies to HTLV-I in the Slovenian population might be somewhere between one in 10 , 000 ( 0.01 % ) and one in 15 , 000 ( 0.0066 % ) , which is similar or even higher to prevalence rates in other European countries .
	manualset3
160464	1	411752	7	NULL	NULL	0	NULL	prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of autism has been estimated as about 0.05 % in the U.S and many European countries , while it was reported to be 0.1 % or higher in Japan and some European countries , though the reasons for this difference are unclear .
	manualset3
160465	2	411752	7	NULL	NULL	0	NULL	autism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of autism has been estimated as about 0.05 % in the U.S and many European countries , while it was reported to be 0.1 % or higher in Japan and some European countries , though the reasons for this difference are unclear .
	manualset3
160466	3	411752	7	NULL	NULL	0	NULL	0.05 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of autism has been estimated as about 0.05 % in the U.S and many European countries , while it was reported to be 0.1 % or higher in Japan and some European countries , though the reasons for this difference are unclear .
	manualset3
160467	4	411752	7	NULL	NULL	0	NULL	U.S	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of autism has been estimated as about 0.05 % in the U.S and many European countries , while it was reported to be 0.1 % or higher in Japan and some European countries , though the reasons for this difference are unclear .
	manualset3
160468	5	411752	7	NULL	NULL	0	NULL	European countries	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of autism has been estimated as about 0.05 % in the U.S and many European countries , while it was reported to be 0.1 % or higher in Japan and some European countries , though the reasons for this difference are unclear .
	manualset3
160469	6	411752	7	NULL	NULL	0	NULL	0.1 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of autism has been estimated as about 0.05 % in the U.S and many European countries , while it was reported to be 0.1 % or higher in Japan and some European countries , though the reasons for this difference are unclear .
	manualset3
160470	7	411752	7	NULL	NULL	0	NULL	Japan	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of autism has been estimated as about 0.05 % in the U.S and many European countries , while it was reported to be 0.1 % or higher in Japan and some European countries , though the reasons for this difference are unclear .
	manualset3
160471	8	411752	7	NULL	NULL	0	NULL	European countries	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of autism has been estimated as about 0.05 % in the U.S and many European countries , while it was reported to be 0.1 % or higher in Japan and some European countries , though the reasons for this difference are unclear .
	manualset3
160472	9	411752	7	NULL	NULL	0	NULL	reasons 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of autism has been estimated as about 0.05 % in the U.S and many European countries , while it was reported to be 0.1 % or higher in Japan and some European countries , though the reasons for this difference are unclear .
	manualset3
169224	10	411752	7	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of autism has been estimated as about 0.05 % in the U.S and many European countries , while it was reported to be 0.1 % or higher in Japan and some European countries , though the reasons for this difference are unclear .
	manualset3
160473	1	411753	7	NULL	NULL	0	NULL	prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of distal tubular acidosis with hyperkalemia is on the increase whilst tubular acidosis with hypokalemia remains rare .
	manualset3
160474	2	411753	7	NULL	NULL	0	NULL	distal tubular acidosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of distal tubular acidosis with hyperkalemia is on the increase whilst tubular acidosis with hypokalemia remains rare .
	manualset3
160475	3	411753	7	NULL	NULL	0	NULL	hyperkalemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of distal tubular acidosis with hyperkalemia is on the increase whilst tubular acidosis with hypokalemia remains rare .
	manualset3
160476	4	411753	7	NULL	NULL	0	NULL	tubular acidosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of distal tubular acidosis with hyperkalemia is on the increase whilst tubular acidosis with hypokalemia remains rare .
	manualset3
160477	5	411753	7	NULL	NULL	0	NULL	hypokalemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of distal tubular acidosis with hyperkalemia is on the increase whilst tubular acidosis with hypokalemia remains rare .
	manualset3
160478	1	411754	7	NULL	NULL	0	NULL	prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of fatalities during anesthesia was 3.4 % ( n = 12 ) over the 5-yr period .
	manualset3
160479	2	411754	7	NULL	NULL	0	NULL	fatalities 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of fatalities during anesthesia was 3.4 % ( n = 12 ) over the 5-yr period .
	manualset3
160480	3	411754	7	NULL	NULL	0	NULL	 anesthesia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of fatalities during anesthesia was 3.4 % ( n = 12 ) over the 5-yr period .
	manualset3
160481	4	411754	7	NULL	NULL	0	NULL	3.4 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of fatalities during anesthesia was 3.4 % ( n = 12 ) over the 5-yr period .
	manualset3
160482	5	411754	7	NULL	NULL	0	NULL	 n = 12	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of fatalities during anesthesia was 3.4 % ( n = 12 ) over the 5-yr period .
	manualset3
160483	6	411754	7	NULL	NULL	0	NULL	 5-yr period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of fatalities during anesthesia was 3.4 % ( n = 12 ) over the 5-yr period .
	manualset3
160484	1	411755	7	NULL	NULL	0	NULL	prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of iron deficiency anemia ( IDA ) increased over the malaria season ( P & lt ; .001 ) .
	manualset3
160485	2	411755	7	NULL	NULL	0	NULL	iron deficiency anemia ( IDA )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of iron deficiency anemia ( IDA ) increased over the malaria season ( P & lt ; .001 ) .
	manualset3
160486	3	411755	7	NULL	NULL	0	NULL	 malaria season	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of iron deficiency anemia ( IDA ) increased over the malaria season ( P & lt ; .001 ) .
	manualset3
160487	4	411755	7	NULL	NULL	0	NULL	 P & lt ; .001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of iron deficiency anemia ( IDA ) increased over the malaria season ( P & lt ; .001 ) .
	manualset3
160488	1	411756	7	NULL	NULL	0	NULL	AREAS COVERED	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	AREAS COVERED : This narrative review covers the treatment options available for IBS-D and focuses on rifaximin .
	manualset3
160489	2	411756	7	NULL	NULL	0	NULL	narrative review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	AREAS COVERED : This narrative review covers the treatment options available for IBS-D and focuses on rifaximin .
	manualset3
160490	3	411756	7	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	AREAS COVERED : This narrative review covers the treatment options available for IBS-D and focuses on rifaximin .
	manualset3
160491	4	411756	7	NULL	NULL	0	NULL	available 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	AREAS COVERED : This narrative review covers the treatment options available for IBS-D and focuses on rifaximin .
	manualset3
160492	5	411756	7	NULL	NULL	0	NULL	IBS-D	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	AREAS COVERED : This narrative review covers the treatment options available for IBS-D and focuses on rifaximin .
	manualset3
160493	6	411756	7	NULL	NULL	0	NULL	rifaximin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	AREAS COVERED : This narrative review covers the treatment options available for IBS-D and focuses on rifaximin .
	manualset3
160494	1	411757	7	NULL	NULL	0	NULL	prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of probable depression was significantly more common in the study group compared with control and referent group ( 28 % vs 5 % and 9.44 % ; P = 0.001 ) .
	manualset3
160495	2	411757	7	NULL	NULL	0	NULL	probable depression 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of probable depression was significantly more common in the study group compared with control and referent group ( 28 % vs 5 % and 9.44 % ; P = 0.001 ) .
	manualset3
160496	3	411757	7	NULL	NULL	0	NULL	study group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of probable depression was significantly more common in the study group compared with control and referent group ( 28 % vs 5 % and 9.44 % ; P = 0.001 ) .
	manualset3
160497	4	411757	7	NULL	NULL	0	NULL	control group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of probable depression was significantly more common in the study group compared with control and referent group ( 28 % vs 5 % and 9.44 % ; P = 0.001 ) .
	manualset3
160498	5	411757	7	NULL	NULL	0	NULL	 referent group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of probable depression was significantly more common in the study group compared with control and referent group ( 28 % vs 5 % and 9.44 % ; P = 0.001 ) .
	manualset3
160499	6	411757	7	NULL	NULL	0	NULL	28 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of probable depression was significantly more common in the study group compared with control and referent group ( 28 % vs 5 % and 9.44 % ; P = 0.001 ) .
	manualset3
160500	7	411757	7	NULL	NULL	0	NULL	 5 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of probable depression was significantly more common in the study group compared with control and referent group ( 28 % vs 5 % and 9.44 % ; P = 0.001 ) .
	manualset3
160501	8	411757	7	NULL	NULL	0	NULL	9.44 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of probable depression was significantly more common in the study group compared with control and referent group ( 28 % vs 5 % and 9.44 % ; P = 0.001 ) .
	manualset3
160502	9	411757	7	NULL	NULL	0	NULL	P = 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of probable depression was significantly more common in the study group compared with control and referent group ( 28 % vs 5 % and 9.44 % ; P = 0.001 ) .
	manualset3
160503	1	411758	7	NULL	NULL	0	NULL	prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of prostatism : a population-based survey of urinary symptoms .
	manualset3
160504	2	411758	7	NULL	NULL	0	NULL	 prostatism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of prostatism : a population-based survey of urinary symptoms .
	manualset3
160505	3	411758	7	NULL	NULL	0	NULL	 population-based survey 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of prostatism : a population-based survey of urinary symptoms .
	manualset3
160506	4	411758	7	NULL	NULL	0	NULL	urinary symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of prostatism : a population-based survey of urinary symptoms .
	manualset3
160507	1	411759	7	NULL	NULL	0	NULL	prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of recent-onset and shortly-before-diagnosed diabetes has been found very high ( 50 % ) in our patients with PC .
	manualset3
160508	2	411759	7	NULL	NULL	0	NULL	recent-onset diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of recent-onset and shortly-before-diagnosed diabetes has been found very high ( 50 % ) in our patients with PC .
	manualset3
160509	3	411759	7	NULL	NULL	0	NULL	shortly-before-diagnosed diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of recent-onset and shortly-before-diagnosed diabetes has been found very high ( 50 % ) in our patients with PC .
	manualset3
160510	4	411759	7	NULL	NULL	0	NULL	50 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of recent-onset and shortly-before-diagnosed diabetes has been found very high ( 50 % ) in our patients with PC .
	manualset3
160511	5	411759	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of recent-onset and shortly-before-diagnosed diabetes has been found very high ( 50 % ) in our patients with PC .
	manualset3
160512	6	411759	7	NULL	NULL	0	NULL	PC	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of recent-onset and shortly-before-diagnosed diabetes has been found very high ( 50 % ) in our patients with PC .
	manualset3
160513	1	411760	7	NULL	NULL	0	NULL	prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of the C/C -13910 - genotype of these young adults did not differ significantly from the corresponding population prevalence of C/C -13910 ( 17.1 % vs 18.1 % ) among Finnish blood donors .
	manualset3
160514	2	411760	7	NULL	NULL	0	NULL	C/C -13910 - genotype	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of the C/C -13910 - genotype of these young adults did not differ significantly from the corresponding population prevalence of C/C -13910 ( 17.1 % vs 18.1 % ) among Finnish blood donors .
	manualset3
160515	3	411760	7	NULL	NULL	0	NULL	young adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of the C/C -13910 - genotype of these young adults did not differ significantly from the corresponding population prevalence of C/C -13910 ( 17.1 % vs 18.1 % ) among Finnish blood donors .
	manualset3
160516	4	411760	7	NULL	NULL	0	NULL	population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of the C/C -13910 - genotype of these young adults did not differ significantly from the corresponding population prevalence of C/C -13910 ( 17.1 % vs 18.1 % ) among Finnish blood donors .
	manualset3
160517	5	411760	7	NULL	NULL	0	NULL	prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of the C/C -13910 - genotype of these young adults did not differ significantly from the corresponding population prevalence of C/C -13910 ( 17.1 % vs 18.1 % ) among Finnish blood donors .
	manualset3
160518	6	411760	7	NULL	NULL	0	NULL	C/C -13910	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of the C/C -13910 - genotype of these young adults did not differ significantly from the corresponding population prevalence of C/C -13910 ( 17.1 % vs 18.1 % ) among Finnish blood donors .
	manualset3
160519	7	411760	7	NULL	NULL	0	NULL	17.1 % vs 18.1 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of the C/C -13910 - genotype of these young adults did not differ significantly from the corresponding population prevalence of C/C -13910 ( 17.1 % vs 18.1 % ) among Finnish blood donors .
	manualset3
160520	8	411760	7	NULL	NULL	0	NULL	Finnish blood donors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of the C/C -13910 - genotype of these young adults did not differ significantly from the corresponding population prevalence of C/C -13910 ( 17.1 % vs 18.1 % ) among Finnish blood donors .
	manualset3
160521	1	411761	7	NULL	NULL	0	NULL	prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of urinary incontinence was found to be nearly the same 8 weeks postpartum as during pregnancy .
	manualset3
160522	2	411761	7	NULL	NULL	0	NULL	 urinary incontinence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of urinary incontinence was found to be nearly the same 8 weeks postpartum as during pregnancy .
	manualset3
160523	3	411761	7	NULL	NULL	0	NULL	8 weeks postpartum	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of urinary incontinence was found to be nearly the same 8 weeks postpartum as during pregnancy .
	manualset3
160524	4	411761	7	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalence of urinary incontinence was found to be nearly the same 8 weeks postpartum as during pregnancy .
	manualset3
160525	1	411762	7	NULL	NULL	0	NULL	prevlances	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalences of CKD , concentric remodeling , eccentric hypertrophy and concentric hypertrophy were significantly increased after 4 years ( all p & lt ; or = 0.033 ) .
	manualset3
160526	2	411762	7	NULL	NULL	0	NULL	CKD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalences of CKD , concentric remodeling , eccentric hypertrophy and concentric hypertrophy were significantly increased after 4 years ( all p & lt ; or = 0.033 ) .
	manualset3
160527	3	411762	7	NULL	NULL	0	NULL	concentric remodeling	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalences of CKD , concentric remodeling , eccentric hypertrophy and concentric hypertrophy were significantly increased after 4 years ( all p & lt ; or = 0.033 ) .
	manualset3
160528	4	411762	7	NULL	NULL	0	NULL	eccentric hypertrophy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalences of CKD , concentric remodeling , eccentric hypertrophy and concentric hypertrophy were significantly increased after 4 years ( all p & lt ; or = 0.033 ) .
	manualset3
160529	5	411762	7	NULL	NULL	0	NULL	concentric hypertrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalences of CKD , concentric remodeling , eccentric hypertrophy and concentric hypertrophy were significantly increased after 4 years ( all p & lt ; or = 0.033 ) .
	manualset3
160530	6	411762	7	NULL	NULL	0	NULL	 4 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalences of CKD , concentric remodeling , eccentric hypertrophy and concentric hypertrophy were significantly increased after 4 years ( all p & lt ; or = 0.033 ) .
	manualset3
160531	7	411762	7	NULL	NULL	0	NULL	p & lt ; or = 0.033	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevalences of CKD , concentric remodeling , eccentric hypertrophy and concentric hypertrophy were significantly increased after 4 years ( all p & lt ; or = 0.033 ) .
	manualset3
160532	1	411763	7	NULL	NULL	0	NULL	scanning electron microscopy study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The previous scanning electron microscopy study of the Hypoderma species suggested that Hypoderma sinense Pleske ( H. sinense ) was different from Hypoderma bovis ( H. bovis ) and Hypoderma lineatum ( H. lineatum ) .
	manualset3
160533	2	411763	7	NULL	NULL	0	NULL	Hypoderma species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The previous scanning electron microscopy study of the Hypoderma species suggested that Hypoderma sinense Pleske ( H. sinense ) was different from Hypoderma bovis ( H. bovis ) and Hypoderma lineatum ( H. lineatum ) .
	manualset3
160534	3	411763	7	NULL	NULL	0	NULL	Hypoderma sinense Pleske ( H. sinense )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The previous scanning electron microscopy study of the Hypoderma species suggested that Hypoderma sinense Pleske ( H. sinense ) was different from Hypoderma bovis ( H. bovis ) and Hypoderma lineatum ( H. lineatum ) .
	manualset3
160535	4	411763	7	NULL	NULL	0	NULL	Hypoderma bovis ( H. bovis )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The previous scanning electron microscopy study of the Hypoderma species suggested that Hypoderma sinense Pleske ( H. sinense ) was different from Hypoderma bovis ( H. bovis ) and Hypoderma lineatum ( H. lineatum ) .
	manualset3
160536	5	411763	7	NULL	NULL	0	NULL	Hypoderma lineatum ( H. lineatum )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The previous scanning electron microscopy study of the Hypoderma species suggested that Hypoderma sinense Pleske ( H. sinense ) was different from Hypoderma bovis ( H. bovis ) and Hypoderma lineatum ( H. lineatum ) .
	manualset3
160537	1	411764	7	NULL	NULL	0	NULL	ARF	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	ARF in the study developed on the background of a light chain proteinuria in patients with hypercalcemia , dehydration , radiocontrast studies , blood loss , surgical interventions , and severe infections .
	manualset3
160538	2	411764	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	ARF in the study developed on the background of a light chain proteinuria in patients with hypercalcemia , dehydration , radiocontrast studies , blood loss , surgical interventions , and severe infections .
	manualset3
160539	3	411764	7	NULL	NULL	0	NULL	light chain proteinuria	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	ARF in the study developed on the background of a light chain proteinuria in patients with hypercalcemia , dehydration , radiocontrast studies , blood loss , surgical interventions , and severe infections .
	manualset3
160540	4	411764	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	ARF in the study developed on the background of a light chain proteinuria in patients with hypercalcemia , dehydration , radiocontrast studies , blood loss , surgical interventions , and severe infections .
	manualset3
160541	5	411764	7	NULL	NULL	0	NULL	hypercalcemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	ARF in the study developed on the background of a light chain proteinuria in patients with hypercalcemia , dehydration , radiocontrast studies , blood loss , surgical interventions , and severe infections .
	manualset3
160542	6	411764	7	NULL	NULL	0	NULL	dehydration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	ARF in the study developed on the background of a light chain proteinuria in patients with hypercalcemia , dehydration , radiocontrast studies , blood loss , surgical interventions , and severe infections .
	manualset3
160543	7	411764	7	NULL	NULL	0	NULL	radiocontrast studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	ARF in the study developed on the background of a light chain proteinuria in patients with hypercalcemia , dehydration , radiocontrast studies , blood loss , surgical interventions , and severe infections .
	manualset3
160544	8	411764	7	NULL	NULL	0	NULL	 blood loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	ARF in the study developed on the background of a light chain proteinuria in patients with hypercalcemia , dehydration , radiocontrast studies , blood loss , surgical interventions , and severe infections .
	manualset3
160545	9	411764	7	NULL	NULL	0	NULL	surgical interventions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	ARF in the study developed on the background of a light chain proteinuria in patients with hypercalcemia , dehydration , radiocontrast studies , blood loss , surgical interventions , and severe infections .
	manualset3
160546	10	411764	7	NULL	NULL	0	NULL	severe infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	ARF in the study developed on the background of a light chain proteinuria in patients with hypercalcemia , dehydration , radiocontrast studies , blood loss , surgical interventions , and severe infections .
	manualset3
160547	1	411765	7	NULL	NULL	0	NULL	leucine aminopeptidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The previously described leucine aminopeptidase , LAP D , consists of at least two isozymes , designated here LAP P and LAP G. In pupae most LAP activity results from LAP P ( pupal ) ; in larvae and adults , in contrast , most LAP activity results from LAP G ( gut ) .
	manualset3
160548	2	411765	7	NULL	NULL	0	NULL	LAP D	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The previously described leucine aminopeptidase , LAP D , consists of at least two isozymes , designated here LAP P and LAP G. In pupae most LAP activity results from LAP P ( pupal ) ; in larvae and adults , in contrast , most LAP activity results from LAP G ( gut ) .
	manualset3
160549	3	411765	7	NULL	NULL	0	NULL	two isozymes	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The previously described leucine aminopeptidase , LAP D , consists of at least two isozymes , designated here LAP P and LAP G. In pupae most LAP activity results from LAP P ( pupal ) ; in larvae and adults , in contrast , most LAP activity results from LAP G ( gut ) .
	manualset3
160550	4	411765	7	NULL	NULL	0	NULL	LAP P 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The previously described leucine aminopeptidase , LAP D , consists of at least two isozymes , designated here LAP P and LAP G. In pupae most LAP activity results from LAP P ( pupal ) ; in larvae and adults , in contrast , most LAP activity results from LAP G ( gut ) .
	manualset3
160551	5	411765	7	NULL	NULL	0	NULL	LAP G	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The previously described leucine aminopeptidase , LAP D , consists of at least two isozymes , designated here LAP P and LAP G. In pupae most LAP activity results from LAP P ( pupal ) ; in larvae and adults , in contrast , most LAP activity results from LAP G ( gut ) .
	manualset3
160552	6	411765	7	NULL	NULL	0	NULL	 pupae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The previously described leucine aminopeptidase , LAP D , consists of at least two isozymes , designated here LAP P and LAP G. In pupae most LAP activity results from LAP P ( pupal ) ; in larvae and adults , in contrast , most LAP activity results from LAP G ( gut ) .
	manualset3
160553	7	411765	7	NULL	NULL	0	NULL	LAP activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The previously described leucine aminopeptidase , LAP D , consists of at least two isozymes , designated here LAP P and LAP G. In pupae most LAP activity results from LAP P ( pupal ) ; in larvae and adults , in contrast , most LAP activity results from LAP G ( gut ) .
	manualset3
160554	8	411765	7	NULL	NULL	0	NULL	LAP P ( pupal )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The previously described leucine aminopeptidase , LAP D , consists of at least two isozymes , designated here LAP P and LAP G. In pupae most LAP activity results from LAP P ( pupal ) ; in larvae and adults , in contrast , most LAP activity results from LAP G ( gut ) .
	manualset3
160555	9	411765	7	NULL	NULL	0	NULL	larvae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The previously described leucine aminopeptidase , LAP D , consists of at least two isozymes , designated here LAP P and LAP G. In pupae most LAP activity results from LAP P ( pupal ) ; in larvae and adults , in contrast , most LAP activity results from LAP G ( gut ) .
	manualset3
160556	10	411765	7	NULL	NULL	0	NULL	adults	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The previously described leucine aminopeptidase , LAP D , consists of at least two isozymes , designated here LAP P and LAP G. In pupae most LAP activity results from LAP P ( pupal ) ; in larvae and adults , in contrast , most LAP activity results from LAP G ( gut ) .
	manualset3
160557	11	411765	7	NULL	NULL	0	NULL	LAP activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The previously described leucine aminopeptidase , LAP D , consists of at least two isozymes , designated here LAP P and LAP G. In pupae most LAP activity results from LAP P ( pupal ) ; in larvae and adults , in contrast , most LAP activity results from LAP G ( gut ) .
	manualset3
160558	12	411765	7	NULL	NULL	0	NULL	LAP G ( gut )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The previously described leucine aminopeptidase , LAP D , consists of at least two isozymes , designated here LAP P and LAP G. In pupae most LAP activity results from LAP P ( pupal ) ; in larvae and adults , in contrast , most LAP activity results from LAP G ( gut ) .
	manualset3
160559	1	411766	7	NULL	NULL	0	NULL	 price paid	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The price paid : manipulation of otolaryngologists by the tobacco industry to obfuscate the emerging truth that smoking causes cancer .
	manualset3
160560	2	411766	7	NULL	NULL	0	NULL	manipulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The price paid : manipulation of otolaryngologists by the tobacco industry to obfuscate the emerging truth that smoking causes cancer .
	manualset3
160561	3	411766	7	NULL	NULL	0	NULL	otolaryngologists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The price paid : manipulation of otolaryngologists by the tobacco industry to obfuscate the emerging truth that smoking causes cancer .
	manualset3
160562	4	411766	7	NULL	NULL	0	NULL	tobacco industry	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The price paid : manipulation of otolaryngologists by the tobacco industry to obfuscate the emerging truth that smoking causes cancer .
	manualset3
160563	5	411766	7	NULL	NULL	0	NULL	smoking	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The price paid : manipulation of otolaryngologists by the tobacco industry to obfuscate the emerging truth that smoking causes cancer .
	manualset3
160564	6	411766	7	NULL	NULL	NULL	NULL	cancer 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The price paid : manipulation of otolaryngologists by the tobacco industry to obfuscate the emerging truth that smoking causes cancer .
	manualset3
169225	7	411766	7	NULL	NULL	0	NULL	emerging truth	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The price paid : manipulation of otolaryngologists by the tobacco industry to obfuscate the emerging truth that smoking causes cancer .
	manualset3
160565	1	411767	7	NULL	NULL	0	NULL	primacy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The primacy of priming in grammatical learning and intervention : a tutorial .
	manualset3
160566	2	411767	7	NULL	NULL	0	NULL	priming	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The primacy of priming in grammatical learning and intervention : a tutorial .
	manualset3
160567	3	411767	7	NULL	NULL	NULL	NULL	grammatical learning	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The primacy of priming in grammatical learning and intervention : a tutorial .
	manualset3
160568	4	411767	7	NULL	NULL	0	NULL	intervention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The primacy of priming in grammatical learning and intervention : a tutorial .
	manualset3
160569	5	411767	7	NULL	NULL	0	NULL	 tutorial	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The primacy of priming in grammatical learning and intervention : a tutorial .
	manualset3
160570	1	411768	7	NULL	NULL	0	NULL	primary aim 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary aim of this study was to evaluate the accuracy of the quantification of deposition .
	manualset3
160571	2	411768	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary aim of this study was to evaluate the accuracy of the quantification of deposition .
	manualset3
160572	3	411768	7	NULL	NULL	0	NULL	accuracy	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary aim of this study was to evaluate the accuracy of the quantification of deposition .
	manualset3
160573	4	411768	7	NULL	NULL	0	NULL	 quantification	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary aim of this study was to evaluate the accuracy of the quantification of deposition .
	manualset3
160574	5	411768	7	NULL	NULL	0	NULL	deposition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary aim of this study was to evaluate the accuracy of the quantification of deposition .
	manualset3
160575	1	411769	7	NULL	NULL	0	NULL	 primary focus	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary focus was tool grinding , but other important processes examined were metal-working , welding , forging , heat treat , engine testing , and diverse-skilled trades work .
	manualset3
160576	2	411769	7	NULL	NULL	0	NULL	tool grinding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary focus was tool grinding , but other important processes examined were metal-working , welding , forging , heat treat , engine testing , and diverse-skilled trades work .
	manualset3
160577	3	411769	7	NULL	NULL	0	NULL	metal-working	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary focus was tool grinding , but other important processes examined were metal-working , welding , forging , heat treat , engine testing , and diverse-skilled trades work .
	manualset3
160578	4	411769	7	NULL	NULL	0	NULL	welding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary focus was tool grinding , but other important processes examined were metal-working , welding , forging , heat treat , engine testing , and diverse-skilled trades work .
	manualset3
160579	5	411769	7	NULL	NULL	0	NULL	forging	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary focus was tool grinding , but other important processes examined were metal-working , welding , forging , heat treat , engine testing , and diverse-skilled trades work .
	manualset3
160580	6	411769	7	NULL	NULL	0	NULL	heat treat	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary focus was tool grinding , but other important processes examined were metal-working , welding , forging , heat treat , engine testing , and diverse-skilled trades work .
	manualset3
160581	7	411769	7	NULL	NULL	0	NULL	engine testing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary focus was tool grinding , but other important processes examined were metal-working , welding , forging , heat treat , engine testing , and diverse-skilled trades work .
	manualset3
160582	8	411769	7	NULL	NULL	0	NULL	diverse-skilled trades work	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary focus was tool grinding , but other important processes examined were metal-working , welding , forging , heat treat , engine testing , and diverse-skilled trades work .
	manualset3
160583	1	411770	7	NULL	NULL	0	NULL	primary neoplasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary neoplasia was detected in 8 patients ( 89 % ) and corresponded to : gastric cancer ( n = 4 ) , colon cancer ( n = 2 ) , gallbladder cancer ( n = 1 ) and breast cancer ( n = 1 ) .
	manualset3
160584	2	411770	7	NULL	NULL	0	NULL	8 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary neoplasia was detected in 8 patients ( 89 % ) and corresponded to : gastric cancer ( n = 4 ) , colon cancer ( n = 2 ) , gallbladder cancer ( n = 1 ) and breast cancer ( n = 1 ) .
	manualset3
160585	3	411770	7	NULL	NULL	0	NULL	89 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary neoplasia was detected in 8 patients ( 89 % ) and corresponded to : gastric cancer ( n = 4 ) , colon cancer ( n = 2 ) , gallbladder cancer ( n = 1 ) and breast cancer ( n = 1 ) .
	manualset3
160586	4	411770	7	NULL	NULL	0	NULL	gastric cancer	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary neoplasia was detected in 8 patients ( 89 % ) and corresponded to : gastric cancer ( n = 4 ) , colon cancer ( n = 2 ) , gallbladder cancer ( n = 1 ) and breast cancer ( n = 1 ) .
	manualset3
160587	5	411770	7	NULL	NULL	0	NULL	n = 4	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary neoplasia was detected in 8 patients ( 89 % ) and corresponded to : gastric cancer ( n = 4 ) , colon cancer ( n = 2 ) , gallbladder cancer ( n = 1 ) and breast cancer ( n = 1 ) .
	manualset3
160588	6	411770	7	NULL	NULL	0	NULL	colon cancer	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary neoplasia was detected in 8 patients ( 89 % ) and corresponded to : gastric cancer ( n = 4 ) , colon cancer ( n = 2 ) , gallbladder cancer ( n = 1 ) and breast cancer ( n = 1 ) .
	manualset3
160589	7	411770	7	NULL	NULL	0	NULL	 n = 2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary neoplasia was detected in 8 patients ( 89 % ) and corresponded to : gastric cancer ( n = 4 ) , colon cancer ( n = 2 ) , gallbladder cancer ( n = 1 ) and breast cancer ( n = 1 ) .
	manualset3
160590	8	411770	7	NULL	NULL	0	NULL	gallbladder cancer	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary neoplasia was detected in 8 patients ( 89 % ) and corresponded to : gastric cancer ( n = 4 ) , colon cancer ( n = 2 ) , gallbladder cancer ( n = 1 ) and breast cancer ( n = 1 ) .
	manualset3
160591	9	411770	7	NULL	NULL	0	NULL	n = 1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary neoplasia was detected in 8 patients ( 89 % ) and corresponded to : gastric cancer ( n = 4 ) , colon cancer ( n = 2 ) , gallbladder cancer ( n = 1 ) and breast cancer ( n = 1 ) .
	manualset3
160592	10	411770	7	NULL	NULL	0	NULL	breast cancer	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary neoplasia was detected in 8 patients ( 89 % ) and corresponded to : gastric cancer ( n = 4 ) , colon cancer ( n = 2 ) , gallbladder cancer ( n = 1 ) and breast cancer ( n = 1 ) .
	manualset3
160593	11	411770	7	NULL	NULL	0	NULL	n = 1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary neoplasia was detected in 8 patients ( 89 % ) and corresponded to : gastric cancer ( n = 4 ) , colon cancer ( n = 2 ) , gallbladder cancer ( n = 1 ) and breast cancer ( n = 1 ) .
	manualset3
160594	1	411771	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary purpose of the present study was to increase our understanding of the roles of chronicity and controllability in the measurement of stress within the context of stress-illness relationships .
	manualset3
160595	2	411771	7	NULL	NULL	NULL	NULL	 study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The primary purpose of the present study was to increase our understanding of the roles of chronicity and controllability in the measurement of stress within the context of stress-illness relationships .
	manualset3
160596	3	411771	7	NULL	NULL	0	NULL	roles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary purpose of the present study was to increase our understanding of the roles of chronicity and controllability in the measurement of stress within the context of stress-illness relationships .
	manualset3
160597	4	411771	7	NULL	NULL	NULL	NULL	chronicity 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The primary purpose of the present study was to increase our understanding of the roles of chronicity and controllability in the measurement of stress within the context of stress-illness relationships .
	manualset3
160598	5	411771	7	NULL	NULL	0	NULL	controllability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary purpose of the present study was to increase our understanding of the roles of chronicity and controllability in the measurement of stress within the context of stress-illness relationships .
	manualset3
160599	6	411771	7	NULL	NULL	0	NULL	measurement	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary purpose of the present study was to increase our understanding of the roles of chronicity and controllability in the measurement of stress within the context of stress-illness relationships .
	manualset3
160600	7	411771	7	NULL	NULL	NULL	NULL	stress	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The primary purpose of the present study was to increase our understanding of the roles of chronicity and controllability in the measurement of stress within the context of stress-illness relationships .
	manualset3
160601	8	411771	7	NULL	NULL	0	NULL	stress-illness relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary purpose of the present study was to increase our understanding of the roles of chronicity and controllability in the measurement of stress within the context of stress-illness relationships .
	manualset3
161707	9	411771	7	NULL	NULL	0	NULL	context	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary purpose of the present study was to increase our understanding of the roles of chronicity and controllability in the measurement of stress within the context of stress-illness relationships .
	manualset3
169226	10	411771	7	NULL	NULL	0	NULL	understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary purpose of the present study was to increase our understanding of the roles of chronicity and controllability in the measurement of stress within the context of stress-illness relationships .
	manualset3
160602	1	411772	7	NULL	NULL	0	NULL	ASHG	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	ASHG statement on genetics and privacy : testimony to United States Congress .
	manualset3
160603	2	411772	7	NULL	NULL	0	NULL	genetics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	ASHG statement on genetics and privacy : testimony to United States Congress .
	manualset3
160604	3	411772	7	NULL	NULL	0	NULL	privacy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	ASHG statement on genetics and privacy : testimony to United States Congress .
	manualset3
160605	4	411772	7	NULL	NULL	0	NULL	testimony	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	ASHG statement on genetics and privacy : testimony to United States Congress .
	manualset3
160606	5	411772	7	NULL	NULL	0	NULL	United States Congress	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	ASHG statement on genetics and privacy : testimony to United States Congress .
	manualset3
160607	1	411773	7	NULL	NULL	0	NULL	factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The principal factors leading to the mPT are elevated levels of intracellular Ca2 + and oxidative stress .
	manualset3
160608	2	411773	7	NULL	NULL	0	NULL	mPT	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The principal factors leading to the mPT are elevated levels of intracellular Ca2 + and oxidative stress .
	manualset3
160609	3	411773	7	NULL	NULL	0	NULL	intracellular Ca2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The principal factors leading to the mPT are elevated levels of intracellular Ca2 + and oxidative stress .
	manualset3
160610	4	411773	7	NULL	NULL	0	NULL	oxidative stress	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The principal factors leading to the mPT are elevated levels of intracellular Ca2 + and oxidative stress .
	manualset3
169227	5	411773	7	NULL	NULL	0	NULL	elevated levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The principal factors leading to the mPT are elevated levels of intracellular Ca2 + and oxidative stress .
	manualset3
160611	1	411774	7	NULL	NULL	0	NULL	 findings 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The principal findings were , first , those associated with the characteristic progressive anemia of the disease , such as extramedullary foci of hemopoietic tissue , lymphoid hyperplasia , and the occurrence of hemosiderin in the liver , spleen , and lymph nodes .
	manualset3
160612	2	411774	7	NULL	NULL	NULL	NULL	 progressive anemia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The principal findings were , first , those associated with the characteristic progressive anemia of the disease , such as extramedullary foci of hemopoietic tissue , lymphoid hyperplasia , and the occurrence of hemosiderin in the liver , spleen , and lymph nodes .
	manualset3
160613	3	411774	7	NULL	NULL	NULL	NULL	disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The principal findings were , first , those associated with the characteristic progressive anemia of the disease , such as extramedullary foci of hemopoietic tissue , lymphoid hyperplasia , and the occurrence of hemosiderin in the liver , spleen , and lymph nodes .
	manualset3
160614	4	411774	7	NULL	NULL	NULL	NULL	extramedullary foci of hemopoietic tissue	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The principal findings were , first , those associated with the characteristic progressive anemia of the disease , such as extramedullary foci of hemopoietic tissue , lymphoid hyperplasia , and the occurrence of hemosiderin in the liver , spleen , and lymph nodes .
	manualset3
160615	5	411774	7	NULL	NULL	0	NULL	 lymphoid hyperplasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The principal findings were , first , those associated with the characteristic progressive anemia of the disease , such as extramedullary foci of hemopoietic tissue , lymphoid hyperplasia , and the occurrence of hemosiderin in the liver , spleen , and lymph nodes .
	manualset3
160616	6	411774	7	NULL	NULL	0	NULL	hemosiderin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The principal findings were , first , those associated with the characteristic progressive anemia of the disease , such as extramedullary foci of hemopoietic tissue , lymphoid hyperplasia , and the occurrence of hemosiderin in the liver , spleen , and lymph nodes .
	manualset3
160617	7	411774	7	NULL	NULL	0	NULL	liver 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The principal findings were , first , those associated with the characteristic progressive anemia of the disease , such as extramedullary foci of hemopoietic tissue , lymphoid hyperplasia , and the occurrence of hemosiderin in the liver , spleen , and lymph nodes .
	manualset3
160618	8	411774	7	NULL	NULL	0	NULL	spleen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The principal findings were , first , those associated with the characteristic progressive anemia of the disease , such as extramedullary foci of hemopoietic tissue , lymphoid hyperplasia , and the occurrence of hemosiderin in the liver , spleen , and lymph nodes .
	manualset3
160619	9	411774	7	NULL	NULL	0	NULL	lymph nodes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The principal findings were , first , those associated with the characteristic progressive anemia of the disease , such as extramedullary foci of hemopoietic tissue , lymphoid hyperplasia , and the occurrence of hemosiderin in the liver , spleen , and lymph nodes .
	manualset3
160620	1	411775	7	NULL	NULL	0	NULL	objective	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The principal objective of this study was to determine and compare the capability of human umbilical vessels of normal and pregnancy-induced hypertensive parturients to produce and to release the endothelial-derived relaxing factor .
	manualset3
160621	2	411775	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The principal objective of this study was to determine and compare the capability of human umbilical vessels of normal and pregnancy-induced hypertensive parturients to produce and to release the endothelial-derived relaxing factor .
	manualset3
160623	4	411775	7	NULL	NULL	0	NULL	capability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The principal objective of this study was to determine and compare the capability of human umbilical vessels of normal and pregnancy-induced hypertensive parturients to produce and to release the endothelial-derived relaxing factor .
	manualset3
160624	5	411775	7	NULL	NULL	0	NULL	human umbilical vessels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The principal objective of this study was to determine and compare the capability of human umbilical vessels of normal and pregnancy-induced hypertensive parturients to produce and to release the endothelial-derived relaxing factor .
	manualset3
160625	6	411775	7	NULL	NULL	0	NULL	normal parturients	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The principal objective of this study was to determine and compare the capability of human umbilical vessels of normal and pregnancy-induced hypertensive parturients to produce and to release the endothelial-derived relaxing factor .
	manualset3
160626	7	411775	7	NULL	NULL	0	NULL	pregnancy-induced hypertensive parturients	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The principal objective of this study was to determine and compare the capability of human umbilical vessels of normal and pregnancy-induced hypertensive parturients to produce and to release the endothelial-derived relaxing factor .
	manualset3
160627	8	411775	7	NULL	NULL	NULL	NULL	endothelial-derived relaxing factor	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The principal objective of this study was to determine and compare the capability of human umbilical vessels of normal and pregnancy-induced hypertensive parturients to produce and to release the endothelial-derived relaxing factor .
	manualset3
160628	1	411776	7	NULL	NULL	0	NULL	objective	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The principal objective of this work has been to determine whether Asn831 of the alpha chain of Na/K-ATPase is located at the cytoplasmic or extracellular surface .
	manualset3
160629	2	411776	7	NULL	NULL	0	NULL	 work	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The principal objective of this work has been to determine whether Asn831 of the alpha chain of Na/K-ATPase is located at the cytoplasmic or extracellular surface .
	manualset3
160630	3	411776	7	NULL	NULL	0	NULL	Asn831	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The principal objective of this work has been to determine whether Asn831 of the alpha chain of Na/K-ATPase is located at the cytoplasmic or extracellular surface .
	manualset3
160631	4	411776	7	NULL	NULL	0	NULL	 alpha chain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The principal objective of this work has been to determine whether Asn831 of the alpha chain of Na/K-ATPase is located at the cytoplasmic or extracellular surface .
	manualset3
160632	5	411776	7	NULL	NULL	0	NULL	Na/K-ATPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The principal objective of this work has been to determine whether Asn831 of the alpha chain of Na/K-ATPase is located at the cytoplasmic or extracellular surface .
	manualset3
160633	6	411776	7	NULL	NULL	NULL	NULL	cytoplasmic surface	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The principal objective of this work has been to determine whether Asn831 of the alpha chain of Na/K-ATPase is located at the cytoplasmic or extracellular surface .
	manualset3
160634	7	411776	7	NULL	NULL	0	NULL	extracellular surface	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The principal objective of this work has been to determine whether Asn831 of the alpha chain of Na/K-ATPase is located at the cytoplasmic or extracellular surface .
	manualset3
160635	1	411777	7	NULL	NULL	0	NULL	principle	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The principle of chemoprevention is based on the fundamental concept that since lung cancer develops through several stages , subjects exposed to risk factors could be given a compound or compounds counteracting the deleterious effect of carcinogenic substances on DNA and/or blocking the subsequent cascade of molecular events .
	manualset3
160636	2	411777	7	NULL	NULL	0	NULL	chemoprevention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The principle of chemoprevention is based on the fundamental concept that since lung cancer develops through several stages , subjects exposed to risk factors could be given a compound or compounds counteracting the deleterious effect of carcinogenic substances on DNA and/or blocking the subsequent cascade of molecular events .
	manualset3
160637	3	411777	7	NULL	NULL	NULL	NULL	fundamental concept	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The principle of chemoprevention is based on the fundamental concept that since lung cancer develops through several stages , subjects exposed to risk factors could be given a compound or compounds counteracting the deleterious effect of carcinogenic substances on DNA and/or blocking the subsequent cascade of molecular events .
	manualset3
160638	4	411777	7	NULL	NULL	NULL	NULL	lung cancer 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The principle of chemoprevention is based on the fundamental concept that since lung cancer develops through several stages , subjects exposed to risk factors could be given a compound or compounds counteracting the deleterious effect of carcinogenic substances on DNA and/or blocking the subsequent cascade of molecular events .
	manualset3
160639	5	411777	7	NULL	NULL	0	NULL	stages	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The principle of chemoprevention is based on the fundamental concept that since lung cancer develops through several stages , subjects exposed to risk factors could be given a compound or compounds counteracting the deleterious effect of carcinogenic substances on DNA and/or blocking the subsequent cascade of molecular events .
	manualset3
160640	6	411777	7	NULL	NULL	0	NULL	subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The principle of chemoprevention is based on the fundamental concept that since lung cancer develops through several stages , subjects exposed to risk factors could be given a compound or compounds counteracting the deleterious effect of carcinogenic substances on DNA and/or blocking the subsequent cascade of molecular events .
	manualset3
160641	7	411777	7	NULL	NULL	0	NULL	risk factors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The principle of chemoprevention is based on the fundamental concept that since lung cancer develops through several stages , subjects exposed to risk factors could be given a compound or compounds counteracting the deleterious effect of carcinogenic substances on DNA and/or blocking the subsequent cascade of molecular events .
	manualset3
160642	8	411777	7	NULL	NULL	0	NULL	 compound 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The principle of chemoprevention is based on the fundamental concept that since lung cancer develops through several stages , subjects exposed to risk factors could be given a compound or compounds counteracting the deleterious effect of carcinogenic substances on DNA and/or blocking the subsequent cascade of molecular events .
	manualset3
160643	9	411777	7	NULL	NULL	0	NULL	compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The principle of chemoprevention is based on the fundamental concept that since lung cancer develops through several stages , subjects exposed to risk factors could be given a compound or compounds counteracting the deleterious effect of carcinogenic substances on DNA and/or blocking the subsequent cascade of molecular events .
	manualset3
160644	10	411777	7	NULL	NULL	0	NULL	deleterious effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The principle of chemoprevention is based on the fundamental concept that since lung cancer develops through several stages , subjects exposed to risk factors could be given a compound or compounds counteracting the deleterious effect of carcinogenic substances on DNA and/or blocking the subsequent cascade of molecular events .
	manualset3
160645	11	411777	7	NULL	NULL	0	NULL	carcinogenic substances	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The principle of chemoprevention is based on the fundamental concept that since lung cancer develops through several stages , subjects exposed to risk factors could be given a compound or compounds counteracting the deleterious effect of carcinogenic substances on DNA and/or blocking the subsequent cascade of molecular events .
	manualset3
160646	12	411777	7	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The principle of chemoprevention is based on the fundamental concept that since lung cancer develops through several stages , subjects exposed to risk factors could be given a compound or compounds counteracting the deleterious effect of carcinogenic substances on DNA and/or blocking the subsequent cascade of molecular events .
	manualset3
160648	14	411777	7	NULL	NULL	0	NULL	molecular events	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The principle of chemoprevention is based on the fundamental concept that since lung cancer develops through several stages , subjects exposed to risk factors could be given a compound or compounds counteracting the deleterious effect of carcinogenic substances on DNA and/or blocking the subsequent cascade of molecular events .
	manualset3
160686	13	411777	7	NULL	NULL	NULL	NULL	cascade	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The principle of chemoprevention is based on the fundamental concept that since lung cancer develops through several stages , subjects exposed to risk factors could be given a compound or compounds counteracting the deleterious effect of carcinogenic substances on DNA and/or blocking the subsequent cascade of molecular events .
	manualset3
160649	1	411778	7	NULL	NULL	0	NULL	principle	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The principle of measurement , construction of transmitter coil assembly , and simple but accurate direct calibration are also described .
	manualset3
160650	2	411778	7	NULL	NULL	0	NULL	measurement	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The principle of measurement , construction of transmitter coil assembly , and simple but accurate direct calibration are also described .
	manualset3
160651	3	411778	7	NULL	NULL	0	NULL	construction of transmitter coil assembly	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The principle of measurement , construction of transmitter coil assembly , and simple but accurate direct calibration are also described .
	manualset3
160652	4	411778	7	NULL	NULL	NULL	NULL	direct calibration	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The principle of measurement , construction of transmitter coil assembly , and simple but accurate direct calibration are also described .
	manualset3
160653	1	411779	7	NULL	NULL	0	NULL	 principle	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The principle of the neutron microbeam is to use the proton beam with a micrometre-sized diameter impinging on a very thin lithium fluoride target system .
	manualset3
160654	2	411779	7	NULL	NULL	0	NULL	neutron microbeam	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The principle of the neutron microbeam is to use the proton beam with a micrometre-sized diameter impinging on a very thin lithium fluoride target system .
	manualset3
160655	3	411779	7	NULL	NULL	0	NULL	proton beam	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The principle of the neutron microbeam is to use the proton beam with a micrometre-sized diameter impinging on a very thin lithium fluoride target system .
	manualset3
160656	4	411779	7	NULL	NULL	0	NULL	micrometre-sized diameter	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The principle of the neutron microbeam is to use the proton beam with a micrometre-sized diameter impinging on a very thin lithium fluoride target system .
	manualset3
160657	5	411779	7	NULL	NULL	NULL	NULL	thin lithium fluoride target system	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The principle of the neutron microbeam is to use the proton beam with a micrometre-sized diameter impinging on a very thin lithium fluoride target system .
	manualset3
160658	1	411780	7	NULL	NULL	0	NULL	principles	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The principles for constructing a minimal , single-chain antigen-binding domain based on one of the digoxin-specific antibodies are also outlined , as are the principles for incorporating such domains into fusion proteins .
	manualset3
160659	2	411780	7	NULL	NULL	0	NULL	single-chain antigen-binding domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The principles for constructing a minimal , single-chain antigen-binding domain based on one of the digoxin-specific antibodies are also outlined , as are the principles for incorporating such domains into fusion proteins .
	manualset3
160660	3	411780	7	NULL	NULL	0	NULL	digoxin-specific antibodies	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The principles for constructing a minimal , single-chain antigen-binding domain based on one of the digoxin-specific antibodies are also outlined , as are the principles for incorporating such domains into fusion proteins .
	manualset3
160661	4	411780	7	NULL	NULL	0	NULL	principles	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The principles for constructing a minimal , single-chain antigen-binding domain based on one of the digoxin-specific antibodies are also outlined , as are the principles for incorporating such domains into fusion proteins .
	manualset3
160662	5	411780	7	NULL	NULL	0	NULL	domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The principles for constructing a minimal , single-chain antigen-binding domain based on one of the digoxin-specific antibodies are also outlined , as are the principles for incorporating such domains into fusion proteins .
	manualset3
160663	6	411780	7	NULL	NULL	0	NULL	fusion proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The principles for constructing a minimal , single-chain antigen-binding domain based on one of the digoxin-specific antibodies are also outlined , as are the principles for incorporating such domains into fusion proteins .
	manualset3
160664	1	411781	7	NULL	NULL	0	NULL	principles	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The principles of physics have been largely de-emphasized in modern medicine in favor of chemistry .
	manualset3
160665	2	411781	7	NULL	NULL	0	NULL	physics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The principles of physics have been largely de-emphasized in modern medicine in favor of chemistry .
	manualset3
160666	3	411781	7	NULL	NULL	0	NULL	modern medicine	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The principles of physics have been largely de-emphasized in modern medicine in favor of chemistry .
	manualset3
160667	4	411781	7	NULL	NULL	0	NULL	chemistry	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The principles of physics have been largely de-emphasized in modern medicine in favor of chemistry .
	manualset3
160668	1	411782	7	NULL	NULL	NULL	NULL	problem	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The problem of differential diagnosis is discussed .
	manualset3
160669	2	411782	7	NULL	NULL	0	NULL	 differential diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The problem of differential diagnosis is discussed .
	manualset3
160670	1	411783	7	NULL	NULL	0	NULL	 problem 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The problem of heredity of the individual disposition for malignant tumors ( immunity and protectivity hypothesis ) is demonstrated by example of a melanom-family .
	manualset3
160671	2	411783	7	NULL	NULL	0	NULL	heredity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The problem of heredity of the individual disposition for malignant tumors ( immunity and protectivity hypothesis ) is demonstrated by example of a melanom-family .
	manualset3
160672	3	411783	7	NULL	NULL	0	NULL	individual disposition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The problem of heredity of the individual disposition for malignant tumors ( immunity and protectivity hypothesis ) is demonstrated by example of a melanom-family .
	manualset3
160673	4	411783	7	NULL	NULL	0	NULL	malignant tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The problem of heredity of the individual disposition for malignant tumors ( immunity and protectivity hypothesis ) is demonstrated by example of a melanom-family .
	manualset3
160674	5	411783	7	NULL	NULL	0	NULL	 immunity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The problem of heredity of the individual disposition for malignant tumors ( immunity and protectivity hypothesis ) is demonstrated by example of a melanom-family .
	manualset3
160675	6	411783	7	NULL	NULL	0	NULL	protectivity hypothesis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The problem of heredity of the individual disposition for malignant tumors ( immunity and protectivity hypothesis ) is demonstrated by example of a melanom-family .
	manualset3
160676	7	411783	7	NULL	NULL	0	NULL	example	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The problem of heredity of the individual disposition for malignant tumors ( immunity and protectivity hypothesis ) is demonstrated by example of a melanom-family .
	manualset3
160677	8	411783	7	NULL	NULL	NULL	NULL	melanom-family	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The problem of heredity of the individual disposition for malignant tumors ( immunity and protectivity hypothesis ) is demonstrated by example of a melanom-family .
	manualset3
160678	1	411784	7	NULL	NULL	0	NULL	problem	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The problem of lifting nonambulatory elderly people has been addressed by means of a modular mobile lifting system that offers the advantage of overhead lifting at lower cost than traditional movement devices for nonambulatory people .
	manualset3
160679	2	411784	7	NULL	NULL	0	NULL	nonambulatory elderly people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The problem of lifting nonambulatory elderly people has been addressed by means of a modular mobile lifting system that offers the advantage of overhead lifting at lower cost than traditional movement devices for nonambulatory people .
	manualset3
160680	3	411784	7	NULL	NULL	0	NULL	modular mobile lifting system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The problem of lifting nonambulatory elderly people has been addressed by means of a modular mobile lifting system that offers the advantage of overhead lifting at lower cost than traditional movement devices for nonambulatory people .
	manualset3
160681	4	411784	7	NULL	NULL	0	NULL	advantage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The problem of lifting nonambulatory elderly people has been addressed by means of a modular mobile lifting system that offers the advantage of overhead lifting at lower cost than traditional movement devices for nonambulatory people .
	manualset3
160682	5	411784	7	NULL	NULL	0	NULL	overhead lifting	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The problem of lifting nonambulatory elderly people has been addressed by means of a modular mobile lifting system that offers the advantage of overhead lifting at lower cost than traditional movement devices for nonambulatory people .
	manualset3
160683	6	411784	7	NULL	NULL	0	NULL	lower cost	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The problem of lifting nonambulatory elderly people has been addressed by means of a modular mobile lifting system that offers the advantage of overhead lifting at lower cost than traditional movement devices for nonambulatory people .
	manualset3
160684	7	411784	7	NULL	NULL	0	NULL	traditional movement devices	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The problem of lifting nonambulatory elderly people has been addressed by means of a modular mobile lifting system that offers the advantage of overhead lifting at lower cost than traditional movement devices for nonambulatory people .
	manualset3
160685	8	411784	7	NULL	NULL	0	NULL	nonambulatory people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The problem of lifting nonambulatory elderly people has been addressed by means of a modular mobile lifting system that offers the advantage of overhead lifting at lower cost than traditional movement devices for nonambulatory people .
	manualset3
169321	9	411784	7	NULL	NULL	0	NULL	means	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The problem of lifting nonambulatory elderly people has been addressed by means of a modular mobile lifting system that offers the advantage of overhead lifting at lower cost than traditional movement devices for nonambulatory people .
	manualset3
160687	1	411785	7	NULL	NULL	0	NULL	problem	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The problem of the postoperative treatment problem is then discussed with special regard to the treatment of shock , the prevention of recurrences and the short intestine syndrome .
	manualset3
160688	2	411785	7	NULL	NULL	0	NULL	postoperative treatment problem	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The problem of the postoperative treatment problem is then discussed with special regard to the treatment of shock , the prevention of recurrences and the short intestine syndrome .
	manualset3
160689	3	411785	7	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The problem of the postoperative treatment problem is then discussed with special regard to the treatment of shock , the prevention of recurrences and the short intestine syndrome .
	manualset3
160690	4	411785	7	NULL	NULL	0	NULL	shock	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The problem of the postoperative treatment problem is then discussed with special regard to the treatment of shock , the prevention of recurrences and the short intestine syndrome .
	manualset3
160691	5	411785	7	NULL	NULL	NULL	NULL	prevention	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The problem of the postoperative treatment problem is then discussed with special regard to the treatment of shock , the prevention of recurrences and the short intestine syndrome .
	manualset3
160692	6	411785	7	NULL	NULL	0	NULL	short intestine syndrome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The problem of the postoperative treatment problem is then discussed with special regard to the treatment of shock , the prevention of recurrences and the short intestine syndrome .
	manualset3
160693	1	411786	7	NULL	NULL	0	NULL	problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The problems about pediatric respiratory management , neonatal emergency surgery and pediatric anesthesia were discussed frequently by doctors in different specialties .
	manualset3
160694	2	411786	7	NULL	NULL	0	NULL	pediatric respiratory management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The problems about pediatric respiratory management , neonatal emergency surgery and pediatric anesthesia were discussed frequently by doctors in different specialties .
	manualset3
160695	3	411786	7	NULL	NULL	0	NULL	neonatal emergency surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The problems about pediatric respiratory management , neonatal emergency surgery and pediatric anesthesia were discussed frequently by doctors in different specialties .
	manualset3
160696	4	411786	7	NULL	NULL	0	NULL	pediatric anesthesia	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The problems about pediatric respiratory management , neonatal emergency surgery and pediatric anesthesia were discussed frequently by doctors in different specialties .
	manualset3
160697	5	411786	7	NULL	NULL	0	NULL	doctors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The problems about pediatric respiratory management , neonatal emergency surgery and pediatric anesthesia were discussed frequently by doctors in different specialties .
	manualset3
169322	6	411786	7	NULL	NULL	0	NULL	specialties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The problems about pediatric respiratory management , neonatal emergency surgery and pediatric anesthesia were discussed frequently by doctors in different specialties .
	manualset3
160698	1	411787	7	NULL	NULL	0	NULL	problems 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The problems of standardization of the AgNOR technique are especially crucial for the retrospective evaluation of fixed and embedded pathological material .
	manualset3
160699	2	411787	7	NULL	NULL	0	NULL	standardization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The problems of standardization of the AgNOR technique are especially crucial for the retrospective evaluation of fixed and embedded pathological material .
	manualset3
160700	3	411787	7	NULL	NULL	0	NULL	AgNOR technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The problems of standardization of the AgNOR technique are especially crucial for the retrospective evaluation of fixed and embedded pathological material .
	manualset3
160701	4	411787	7	NULL	NULL	0	NULL	evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The problems of standardization of the AgNOR technique are especially crucial for the retrospective evaluation of fixed and embedded pathological material .
	manualset3
160702	5	411787	7	NULL	NULL	0	NULL	fixed pathological material	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The problems of standardization of the AgNOR technique are especially crucial for the retrospective evaluation of fixed and embedded pathological material .
	manualset3
160703	6	411787	7	NULL	NULL	0	NULL	embedded pathological material 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The problems of standardization of the AgNOR technique are especially crucial for the retrospective evaluation of fixed and embedded pathological material .
	manualset3
160704	1	411788	7	NULL	NULL	0	NULL	problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The problems of vaccination against smallpox ( Hebrew Text ) .
	manualset3
160705	2	411788	7	NULL	NULL	0	NULL	vaccination 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The problems of vaccination against smallpox ( Hebrew Text ) .
	manualset3
160706	3	411788	7	NULL	NULL	NULL	NULL	smallpox	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The problems of vaccination against smallpox ( Hebrew Text ) .
	manualset3
160707	4	411788	7	NULL	NULL	0	NULL	Hebrew Text	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The problems of vaccination against smallpox ( Hebrew Text ) .
	manualset3
160708	1	411789	7	NULL	NULL	0	NULL	procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The procedure failed in four patients , for a failure rate of 3.7 % ; three of these failures occurred more than 12 months after sterilization .
	manualset3
160709	2	411789	7	NULL	NULL	0	NULL	four patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The procedure failed in four patients , for a failure rate of 3.7 % ; three of these failures occurred more than 12 months after sterilization .
	manualset3
160710	3	411789	7	NULL	NULL	0	NULL	failure rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The procedure failed in four patients , for a failure rate of 3.7 % ; three of these failures occurred more than 12 months after sterilization .
	manualset3
160711	4	411789	7	NULL	NULL	0	NULL	3.7 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The procedure failed in four patients , for a failure rate of 3.7 % ; three of these failures occurred more than 12 months after sterilization .
	manualset3
160712	5	411789	7	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The procedure failed in four patients , for a failure rate of 3.7 % ; three of these failures occurred more than 12 months after sterilization .
	manualset3
160713	6	411789	7	NULL	NULL	0	NULL	failures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The procedure failed in four patients , for a failure rate of 3.7 % ; three of these failures occurred more than 12 months after sterilization .
	manualset3
160714	7	411789	7	NULL	NULL	0	NULL	12 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The procedure failed in four patients , for a failure rate of 3.7 % ; three of these failures occurred more than 12 months after sterilization .
	manualset3
160715	8	411789	7	NULL	NULL	0	NULL	sterilization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The procedure failed in four patients , for a failure rate of 3.7 % ; three of these failures occurred more than 12 months after sterilization .
	manualset3
160716	1	411790	7	NULL	NULL	0	NULL	procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The procedure had no side-effect on liver or kidney function .
	manualset3
160717	2	411790	7	NULL	NULL	0	NULL	 side-effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The procedure had no side-effect on liver or kidney function .
	manualset3
160718	3	411790	7	NULL	NULL	NULL	NULL	liver function	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The procedure had no side-effect on liver or kidney function .
	manualset3
160719	4	411790	7	NULL	NULL	0	NULL	kidney function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The procedure had no side-effect on liver or kidney function .
	manualset3
160720	1	411791	7	NULL	NULL	0	NULL	ASYMPTOMATIC MILD INTERMITTENT PROTEINURIA	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	ASYMPTOMATIC MILD INTERMITTENT PROTEINURIA ; A PERCUTANEOUS RENAL BIOPSY STUDY .
	manualset3
160721	2	411791	7	NULL	NULL	0	NULL	PERCUTANEOUS RENAL BIOPSY STUDY	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	ASYMPTOMATIC MILD INTERMITTENT PROTEINURIA ; A PERCUTANEOUS RENAL BIOPSY STUDY .
	manualset3
160722	1	411792	7	NULL	NULL	0	NULL	procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The procedure has a high success rate and has stood the test of time ( over a quarter of a century ) .
	manualset3
160723	2	411792	7	NULL	NULL	0	NULL	success rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The procedure has a high success rate and has stood the test of time ( over a quarter of a century ) .
	manualset3
160724	3	411792	7	NULL	NULL	0	NULL	test of time	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The procedure has a high success rate and has stood the test of time ( over a quarter of a century ) .
	manualset3
160725	4	411792	7	NULL	NULL	0	NULL	quarter of a century	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The procedure has a high success rate and has stood the test of time ( over a quarter of a century ) .
	manualset3
160726	1	411793	7	NULL	NULL	0	NULL	procedure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The procedure is based on the activation of human B cells in microwells by murine thymoma EL4B5 cells .
	manualset3
160727	2	411793	7	NULL	NULL	0	NULL	activation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The procedure is based on the activation of human B cells in microwells by murine thymoma EL4B5 cells .
	manualset3
160728	3	411793	7	NULL	NULL	0	NULL	human B cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The procedure is based on the activation of human B cells in microwells by murine thymoma EL4B5 cells .
	manualset3
160729	4	411793	7	NULL	NULL	0	NULL	microwells	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The procedure is based on the activation of human B cells in microwells by murine thymoma EL4B5 cells .
	manualset3
160730	5	411793	7	NULL	NULL	0	NULL	murine thymoma EL4B5 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The procedure is based on the activation of human B cells in microwells by murine thymoma EL4B5 cells .
	manualset3
160731	1	411794	7	NULL	NULL	0	NULL	 procedure 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The procedure is simple and provides material suitable for physiological studies .
	manualset3
160733	3	411794	7	NULL	NULL	0	NULL	 material 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The procedure is simple and provides material suitable for physiological studies .
	manualset3
160734	4	411794	7	NULL	NULL	0	NULL	physiological studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The procedure is simple and provides material suitable for physiological studies .
	manualset3
160735	1	411795	7	NULL	NULL	0	NULL	procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The procedure may prolong survival , but this has not been proved .
	manualset3
160736	2	411795	7	NULL	NULL	0	NULL	survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The procedure may prolong survival , but this has not been proved .
	manualset3
160737	1	411796	7	NULL	NULL	0	NULL	process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The process applied to a raw source of collagen , bovine pericardium , provided a sponge-like structure , with heterogeneous pore size , and , moreover , the complete removal of interstitial cells .
	manualset3
160738	2	411796	7	NULL	NULL	0	NULL	raw source	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The process applied to a raw source of collagen , bovine pericardium , provided a sponge-like structure , with heterogeneous pore size , and , moreover , the complete removal of interstitial cells .
	manualset3
160739	3	411796	7	NULL	NULL	0	NULL	collagen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The process applied to a raw source of collagen , bovine pericardium , provided a sponge-like structure , with heterogeneous pore size , and , moreover , the complete removal of interstitial cells .
	manualset3
160740	4	411796	7	NULL	NULL	0	NULL	bovine pericardium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The process applied to a raw source of collagen , bovine pericardium , provided a sponge-like structure , with heterogeneous pore size , and , moreover , the complete removal of interstitial cells .
	manualset3
160741	5	411796	7	NULL	NULL	NULL	NULL	sponge-like structure	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The process applied to a raw source of collagen , bovine pericardium , provided a sponge-like structure , with heterogeneous pore size , and , moreover , the complete removal of interstitial cells .
	manualset3
160742	6	411796	7	NULL	NULL	0	NULL	heterogeneous pore size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The process applied to a raw source of collagen , bovine pericardium , provided a sponge-like structure , with heterogeneous pore size , and , moreover , the complete removal of interstitial cells .
	manualset3
160743	7	411796	7	NULL	NULL	0	NULL	removal 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The process applied to a raw source of collagen , bovine pericardium , provided a sponge-like structure , with heterogeneous pore size , and , moreover , the complete removal of interstitial cells .
	manualset3
160744	8	411796	7	NULL	NULL	0	NULL	 interstitial cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The process applied to a raw source of collagen , bovine pericardium , provided a sponge-like structure , with heterogeneous pore size , and , moreover , the complete removal of interstitial cells .
	manualset3
160745	1	411797	7	NULL	NULL	0	NULL	gammagamma	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The process gammagamma -- ) phiJ/psi is measured using a data sample of 825 fb { -1 } collected with the Belle detector .
	manualset3
160746	2	411797	7	NULL	NULL	0	NULL	phiJ/psi	Unit												NULL		0	NULL	NULL	NULL	NULL	NULL	The process gammagamma -- ) phiJ/psi is measured using a data sample of 825 fb { -1 } collected with the Belle detector .
	manualset3
160747	3	411797	7	NULL	NULL	0	NULL	data sample	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The process gammagamma -- ) phiJ/psi is measured using a data sample of 825 fb { -1 } collected with the Belle detector .
	manualset3
160748	4	411797	7	NULL	NULL	0	NULL	825 fb { -1 }	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The process gammagamma -- ) phiJ/psi is measured using a data sample of 825 fb { -1 } collected with the Belle detector .
	manualset3
160749	5	411797	7	NULL	NULL	NULL	NULL	Belle detector	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The process gammagamma -- ) phiJ/psi is measured using a data sample of 825 fb { -1 } collected with the Belle detector .
	manualset3
160750	1	411798	7	NULL	NULL	0	NULL	process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The process of hES cells self-renewal appears to be regulated by many different pathways ; however , the molecular mechanisms enabling this process are not fully characterized .
	manualset3
160751	2	411798	7	NULL	NULL	NULL	NULL	hES cells self-renewal	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The process of hES cells self-renewal appears to be regulated by many different pathways ; however , the molecular mechanisms enabling this process are not fully characterized .
	manualset3
160753	4	411798	7	NULL	NULL	NULL	NULL	pathways	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The process of hES cells self-renewal appears to be regulated by many different pathways ; however , the molecular mechanisms enabling this process are not fully characterized .
	manualset3
160754	5	411798	7	NULL	NULL	0	NULL	molecular mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The process of hES cells self-renewal appears to be regulated by many different pathways ; however , the molecular mechanisms enabling this process are not fully characterized .
	manualset3
160755	6	411798	7	NULL	NULL	0	NULL	process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The process of hES cells self-renewal appears to be regulated by many different pathways ; however , the molecular mechanisms enabling this process are not fully characterized .
	manualset3
160756	1	411799	7	NULL	NULL	0	NULL	process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The process of healing was studied by histological examination .
	manualset3
160757	2	411799	7	NULL	NULL	NULL	NULL	healing	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The process of healing was studied by histological examination .
	manualset3
160758	3	411799	7	NULL	NULL	0	NULL	histological examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The process of healing was studied by histological examination .
	manualset3
160759	1	411800	7	NULL	NULL	0	NULL	process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The process of identifying and understanding cytokines : from basic studies to treating rheumatic diseases .
	manualset3
160760	2	411800	7	NULL	NULL	0	NULL	cytokines	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The process of identifying and understanding cytokines : from basic studies to treating rheumatic diseases .
	manualset3
160761	3	411800	7	NULL	NULL	0	NULL	basic studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The process of identifying and understanding cytokines : from basic studies to treating rheumatic diseases .
	manualset3
160762	4	411800	7	NULL	NULL	0	NULL	rheumatic diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The process of identifying and understanding cytokines : from basic studies to treating rheumatic diseases .
	manualset3
160763	1	411801	7	NULL	NULL	0	NULL	process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The process was partially mediated by CD4 + T cells and by interleukin-4 ( IL-4 ) production , did not require eosinophils , and was independent of gamma interferon ( IFN - ) and IL-17 .
	manualset3
160764	2	411801	7	NULL	NULL	0	NULL	CD4 + T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The process was partially mediated by CD4 + T cells and by interleukin-4 ( IL-4 ) production , did not require eosinophils , and was independent of gamma interferon ( IFN - ) and IL-17 .
	manualset3
160765	3	411801	7	NULL	NULL	0	NULL	interleukin-4 ( IL-4 ) production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The process was partially mediated by CD4 + T cells and by interleukin-4 ( IL-4 ) production , did not require eosinophils , and was independent of gamma interferon ( IFN - ) and IL-17 .
	manualset3
160766	4	411801	7	NULL	NULL	0	NULL	eosinophils	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The process was partially mediated by CD4 + T cells and by interleukin-4 ( IL-4 ) production , did not require eosinophils , and was independent of gamma interferon ( IFN - ) and IL-17 .
	manualset3
160767	5	411801	7	NULL	NULL	0	NULL	gamma interferon ( IFN - )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The process was partially mediated by CD4 + T cells and by interleukin-4 ( IL-4 ) production , did not require eosinophils , and was independent of gamma interferon ( IFN - ) and IL-17 .
	manualset3
160768	6	411801	7	NULL	NULL	0	NULL	IL-17	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The process was partially mediated by CD4 + T cells and by interleukin-4 ( IL-4 ) production , did not require eosinophils , and was independent of gamma interferon ( IFN - ) and IL-17 .
	manualset3
160769	1	411802	7	NULL	NULL	0	NULL	ATBF1 protein levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	ATBF1 protein levels fluctuate with estrogen levels .
	manualset3
160770	2	411802	7	NULL	NULL	0	NULL	estrogen levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	ATBF1 protein levels fluctuate with estrogen levels .
	manualset3
160771	1	411803	7	NULL	NULL	NULL	NULL	product ( 11C ) diazomethane	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The product ( 11C ) diazomethane was measured indirectly in the form of 4-nitrobenzoic acid ( 11C ) methylester using the esterification of 4-nitrobenzoic acid as a monitor reaction .
	manualset3
160772	2	411803	7	NULL	NULL	NULL	NULL	form	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The product ( 11C ) diazomethane was measured indirectly in the form of 4-nitrobenzoic acid ( 11C ) methylester using the esterification of 4-nitrobenzoic acid as a monitor reaction .
	manualset3
160773	3	411803	7	NULL	NULL	0	NULL	 4-nitrobenzoic acid ( 11C ) methylester	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The product ( 11C ) diazomethane was measured indirectly in the form of 4-nitrobenzoic acid ( 11C ) methylester using the esterification of 4-nitrobenzoic acid as a monitor reaction .
	manualset3
160774	4	411803	7	NULL	NULL	0	NULL	esterification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The product ( 11C ) diazomethane was measured indirectly in the form of 4-nitrobenzoic acid ( 11C ) methylester using the esterification of 4-nitrobenzoic acid as a monitor reaction .
	manualset3
160775	5	411803	7	NULL	NULL	0	NULL	4-nitrobenzoic acid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The product ( 11C ) diazomethane was measured indirectly in the form of 4-nitrobenzoic acid ( 11C ) methylester using the esterification of 4-nitrobenzoic acid as a monitor reaction .
	manualset3
160776	6	411803	7	NULL	NULL	0	NULL	monitor reaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The product ( 11C ) diazomethane was measured indirectly in the form of 4-nitrobenzoic acid ( 11C ) methylester using the esterification of 4-nitrobenzoic acid as a monitor reaction .
	manualset3
160777	1	411804	7	NULL	NULL	0	NULL	product	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The product can easily be transformed into a beta ( 2 ) - homoamino acid .
	manualset3
160779	2	411804	7	NULL	NULL	0	NULL	beta ( 2 ) - homoamino acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The product can easily be transformed into a beta ( 2 ) - homoamino acid .
	manualset3
160780	1	411805	7	NULL	NULL	0	NULL	product inhibition patterns	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The product inhibition patterns and addition data are consistent with a reaction mechanism involving an ordered binding of Fe2 + , alpha-ketoglutarate , O2 and the peptide substrate to the enzyme in this order , and an ordered release of the hydroxylated peptide , CO2 , succinate and Fe2 + , in which Fe2 + need not leave the enzyme during each catalytic cycle and in which the order of release of the hydroxylated peptide and CO2 is uncertain .
	manualset3
160781	2	411805	7	NULL	NULL	0	NULL	addition data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The product inhibition patterns and addition data are consistent with a reaction mechanism involving an ordered binding of Fe2 + , alpha-ketoglutarate , O2 and the peptide substrate to the enzyme in this order , and an ordered release of the hydroxylated peptide , CO2 , succinate and Fe2 + , in which Fe2 + need not leave the enzyme during each catalytic cycle and in which the order of release of the hydroxylated peptide and CO2 is uncertain .
	manualset3
160782	3	411805	7	NULL	NULL	0	NULL	reaction mechanism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The product inhibition patterns and addition data are consistent with a reaction mechanism involving an ordered binding of Fe2 + , alpha-ketoglutarate , O2 and the peptide substrate to the enzyme in this order , and an ordered release of the hydroxylated peptide , CO2 , succinate and Fe2 + , in which Fe2 + need not leave the enzyme during each catalytic cycle and in which the order of release of the hydroxylated peptide and CO2 is uncertain .
	manualset3
160784	5	411805	7	NULL	NULL	NULL	NULL	Fe2 +	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The product inhibition patterns and addition data are consistent with a reaction mechanism involving an ordered binding of Fe2 + , alpha-ketoglutarate , O2 and the peptide substrate to the enzyme in this order , and an ordered release of the hydroxylated peptide , CO2 , succinate and Fe2 + , in which Fe2 + need not leave the enzyme during each catalytic cycle and in which the order of release of the hydroxylated peptide and CO2 is uncertain .
	manualset3
160785	6	411805	7	NULL	NULL	0	NULL	alpha-ketoglutarate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The product inhibition patterns and addition data are consistent with a reaction mechanism involving an ordered binding of Fe2 + , alpha-ketoglutarate , O2 and the peptide substrate to the enzyme in this order , and an ordered release of the hydroxylated peptide , CO2 , succinate and Fe2 + , in which Fe2 + need not leave the enzyme during each catalytic cycle and in which the order of release of the hydroxylated peptide and CO2 is uncertain .
	manualset3
160786	7	411805	7	NULL	NULL	0	NULL	O2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The product inhibition patterns and addition data are consistent with a reaction mechanism involving an ordered binding of Fe2 + , alpha-ketoglutarate , O2 and the peptide substrate to the enzyme in this order , and an ordered release of the hydroxylated peptide , CO2 , succinate and Fe2 + , in which Fe2 + need not leave the enzyme during each catalytic cycle and in which the order of release of the hydroxylated peptide and CO2 is uncertain .
	manualset3
160787	8	411805	7	NULL	NULL	0	NULL	peptide substrate	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The product inhibition patterns and addition data are consistent with a reaction mechanism involving an ordered binding of Fe2 + , alpha-ketoglutarate , O2 and the peptide substrate to the enzyme in this order , and an ordered release of the hydroxylated peptide , CO2 , succinate and Fe2 + , in which Fe2 + need not leave the enzyme during each catalytic cycle and in which the order of release of the hydroxylated peptide and CO2 is uncertain .
	manualset3
160788	9	411805	7	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The product inhibition patterns and addition data are consistent with a reaction mechanism involving an ordered binding of Fe2 + , alpha-ketoglutarate , O2 and the peptide substrate to the enzyme in this order , and an ordered release of the hydroxylated peptide , CO2 , succinate and Fe2 + , in which Fe2 + need not leave the enzyme during each catalytic cycle and in which the order of release of the hydroxylated peptide and CO2 is uncertain .
	manualset3
160789	10	411805	7	NULL	NULL	0	NULL	release 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The product inhibition patterns and addition data are consistent with a reaction mechanism involving an ordered binding of Fe2 + , alpha-ketoglutarate , O2 and the peptide substrate to the enzyme in this order , and an ordered release of the hydroxylated peptide , CO2 , succinate and Fe2 + , in which Fe2 + need not leave the enzyme during each catalytic cycle and in which the order of release of the hydroxylated peptide and CO2 is uncertain .
	manualset3
160790	11	411805	7	NULL	NULL	0	NULL	 hydroxylated peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The product inhibition patterns and addition data are consistent with a reaction mechanism involving an ordered binding of Fe2 + , alpha-ketoglutarate , O2 and the peptide substrate to the enzyme in this order , and an ordered release of the hydroxylated peptide , CO2 , succinate and Fe2 + , in which Fe2 + need not leave the enzyme during each catalytic cycle and in which the order of release of the hydroxylated peptide and CO2 is uncertain .
	manualset3
160791	12	411805	7	NULL	NULL	0	NULL	CO2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The product inhibition patterns and addition data are consistent with a reaction mechanism involving an ordered binding of Fe2 + , alpha-ketoglutarate , O2 and the peptide substrate to the enzyme in this order , and an ordered release of the hydroxylated peptide , CO2 , succinate and Fe2 + , in which Fe2 + need not leave the enzyme during each catalytic cycle and in which the order of release of the hydroxylated peptide and CO2 is uncertain .
	manualset3
160792	13	411805	7	NULL	NULL	0	NULL	succinate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The product inhibition patterns and addition data are consistent with a reaction mechanism involving an ordered binding of Fe2 + , alpha-ketoglutarate , O2 and the peptide substrate to the enzyme in this order , and an ordered release of the hydroxylated peptide , CO2 , succinate and Fe2 + , in which Fe2 + need not leave the enzyme during each catalytic cycle and in which the order of release of the hydroxylated peptide and CO2 is uncertain .
	manualset3
160793	14	411805	7	NULL	NULL	NULL	NULL	Fe2 +	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The product inhibition patterns and addition data are consistent with a reaction mechanism involving an ordered binding of Fe2 + , alpha-ketoglutarate , O2 and the peptide substrate to the enzyme in this order , and an ordered release of the hydroxylated peptide , CO2 , succinate and Fe2 + , in which Fe2 + need not leave the enzyme during each catalytic cycle and in which the order of release of the hydroxylated peptide and CO2 is uncertain .
	manualset3
160794	15	411805	7	NULL	NULL	NULL	NULL	Fe2 +	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The product inhibition patterns and addition data are consistent with a reaction mechanism involving an ordered binding of Fe2 + , alpha-ketoglutarate , O2 and the peptide substrate to the enzyme in this order , and an ordered release of the hydroxylated peptide , CO2 , succinate and Fe2 + , in which Fe2 + need not leave the enzyme during each catalytic cycle and in which the order of release of the hydroxylated peptide and CO2 is uncertain .
	manualset3
160795	16	411805	7	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The product inhibition patterns and addition data are consistent with a reaction mechanism involving an ordered binding of Fe2 + , alpha-ketoglutarate , O2 and the peptide substrate to the enzyme in this order , and an ordered release of the hydroxylated peptide , CO2 , succinate and Fe2 + , in which Fe2 + need not leave the enzyme during each catalytic cycle and in which the order of release of the hydroxylated peptide and CO2 is uncertain .
	manualset3
160796	17	411805	7	NULL	NULL	0	NULL	catalytic cycle 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The product inhibition patterns and addition data are consistent with a reaction mechanism involving an ordered binding of Fe2 + , alpha-ketoglutarate , O2 and the peptide substrate to the enzyme in this order , and an ordered release of the hydroxylated peptide , CO2 , succinate and Fe2 + , in which Fe2 + need not leave the enzyme during each catalytic cycle and in which the order of release of the hydroxylated peptide and CO2 is uncertain .
	manualset3
160797	18	411805	7	NULL	NULL	0	NULL	order	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The product inhibition patterns and addition data are consistent with a reaction mechanism involving an ordered binding of Fe2 + , alpha-ketoglutarate , O2 and the peptide substrate to the enzyme in this order , and an ordered release of the hydroxylated peptide , CO2 , succinate and Fe2 + , in which Fe2 + need not leave the enzyme during each catalytic cycle and in which the order of release of the hydroxylated peptide and CO2 is uncertain .
	manualset3
160798	19	411805	7	NULL	NULL	0	NULL	release	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The product inhibition patterns and addition data are consistent with a reaction mechanism involving an ordered binding of Fe2 + , alpha-ketoglutarate , O2 and the peptide substrate to the enzyme in this order , and an ordered release of the hydroxylated peptide , CO2 , succinate and Fe2 + , in which Fe2 + need not leave the enzyme during each catalytic cycle and in which the order of release of the hydroxylated peptide and CO2 is uncertain .
	manualset3
160799	20	411805	7	NULL	NULL	0	NULL	hydroxylated peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The product inhibition patterns and addition data are consistent with a reaction mechanism involving an ordered binding of Fe2 + , alpha-ketoglutarate , O2 and the peptide substrate to the enzyme in this order , and an ordered release of the hydroxylated peptide , CO2 , succinate and Fe2 + , in which Fe2 + need not leave the enzyme during each catalytic cycle and in which the order of release of the hydroxylated peptide and CO2 is uncertain .
	manualset3
160800	21	411805	7	NULL	NULL	0	NULL	CO2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The product inhibition patterns and addition data are consistent with a reaction mechanism involving an ordered binding of Fe2 + , alpha-ketoglutarate , O2 and the peptide substrate to the enzyme in this order , and an ordered release of the hydroxylated peptide , CO2 , succinate and Fe2 + , in which Fe2 + need not leave the enzyme during each catalytic cycle and in which the order of release of the hydroxylated peptide and CO2 is uncertain .
	manualset3
160801	1	411806	7	NULL	NULL	0	NULL	product	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The product of the intron - gene is a more efficient suppressor than the product of an intron + gene .
	manualset3
160802	2	411806	7	NULL	NULL	0	NULL	intron - gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The product of the intron - gene is a more efficient suppressor than the product of an intron + gene .
	manualset3
160803	3	411806	7	NULL	NULL	0	NULL	suppressor	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The product of the intron - gene is a more efficient suppressor than the product of an intron + gene .
	manualset3
160804	4	411806	7	NULL	NULL	0	NULL	product	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The product of the intron - gene is a more efficient suppressor than the product of an intron + gene .
	manualset3
160805	5	411806	7	NULL	NULL	0	NULL	intron + gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The product of the intron - gene is a more efficient suppressor than the product of an intron + gene .
	manualset3
160806	1	411807	7	NULL	NULL	0	NULL	production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The production of choline and phosphatidylethanol stimulated by angiotensin II was completely blocked by the angiotensin II AT1 receptor-selective antagonist DuP 753 with an IC50 value of 8 nM , but not by the angiotensin II AT2 receptor selective ligand CGP 42112A .
	manualset3
160807	2	411807	7	NULL	NULL	0	NULL	choline	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The production of choline and phosphatidylethanol stimulated by angiotensin II was completely blocked by the angiotensin II AT1 receptor-selective antagonist DuP 753 with an IC50 value of 8 nM , but not by the angiotensin II AT2 receptor selective ligand CGP 42112A .
	manualset3
160808	3	411807	7	NULL	NULL	0	NULL	phosphatidylethanol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The production of choline and phosphatidylethanol stimulated by angiotensin II was completely blocked by the angiotensin II AT1 receptor-selective antagonist DuP 753 with an IC50 value of 8 nM , but not by the angiotensin II AT2 receptor selective ligand CGP 42112A .
	manualset3
160809	4	411807	7	NULL	NULL	0	NULL	angiotensin II	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The production of choline and phosphatidylethanol stimulated by angiotensin II was completely blocked by the angiotensin II AT1 receptor-selective antagonist DuP 753 with an IC50 value of 8 nM , but not by the angiotensin II AT2 receptor selective ligand CGP 42112A .
	manualset3
160810	5	411807	7	NULL	NULL	0	NULL	angiotensin II AT1 receptor-selective antagonist DuP 753	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The production of choline and phosphatidylethanol stimulated by angiotensin II was completely blocked by the angiotensin II AT1 receptor-selective antagonist DuP 753 with an IC50 value of 8 nM , but not by the angiotensin II AT2 receptor selective ligand CGP 42112A .
	manualset3
160811	6	411807	7	NULL	NULL	0	NULL	IC50 value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The production of choline and phosphatidylethanol stimulated by angiotensin II was completely blocked by the angiotensin II AT1 receptor-selective antagonist DuP 753 with an IC50 value of 8 nM , but not by the angiotensin II AT2 receptor selective ligand CGP 42112A .
	manualset3
160812	7	411807	7	NULL	NULL	0	NULL	8 nM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The production of choline and phosphatidylethanol stimulated by angiotensin II was completely blocked by the angiotensin II AT1 receptor-selective antagonist DuP 753 with an IC50 value of 8 nM , but not by the angiotensin II AT2 receptor selective ligand CGP 42112A .
	manualset3
160813	8	411807	7	NULL	NULL	0	NULL	angiotensin II AT2 receptor selective ligand CGP 42112A	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The production of choline and phosphatidylethanol stimulated by angiotensin II was completely blocked by the angiotensin II AT1 receptor-selective antagonist DuP 753 with an IC50 value of 8 nM , but not by the angiotensin II AT2 receptor selective ligand CGP 42112A .
	manualset3
160814	1	411808	7	NULL	NULL	0	NULL	production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The production of migration inhibitory factor in response to suboptimal concentrations of Candida , Trichophyton-Oidiomyces-Epidermophyton and mumps virus was not enhanced in either group after 24 hours ' preculture apart from a slight increase in response to mumps virus in the patients .
	manualset3
160815	2	411808	7	NULL	NULL	0	NULL	migration inhibitory factor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The production of migration inhibitory factor in response to suboptimal concentrations of Candida , Trichophyton-Oidiomyces-Epidermophyton and mumps virus was not enhanced in either group after 24 hours ' preculture apart from a slight increase in response to mumps virus in the patients .
	manualset3
160817	3	411808	7	NULL	NULL	0	NULL	Candida	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The production of migration inhibitory factor in response to suboptimal concentrations of Candida , Trichophyton-Oidiomyces-Epidermophyton and mumps virus was not enhanced in either group after 24 hours ' preculture apart from a slight increase in response to mumps virus in the patients .
	manualset3
160818	4	411808	7	NULL	NULL	0	NULL	Trichophyton-Oidiomyces-Epidermophyton	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The production of migration inhibitory factor in response to suboptimal concentrations of Candida , Trichophyton-Oidiomyces-Epidermophyton and mumps virus was not enhanced in either group after 24 hours ' preculture apart from a slight increase in response to mumps virus in the patients .
	manualset3
160819	5	411808	7	NULL	NULL	0	NULL	mumps virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The production of migration inhibitory factor in response to suboptimal concentrations of Candida , Trichophyton-Oidiomyces-Epidermophyton and mumps virus was not enhanced in either group after 24 hours ' preculture apart from a slight increase in response to mumps virus in the patients .
	manualset3
160820	6	411808	7	NULL	NULL	0	NULL	group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The production of migration inhibitory factor in response to suboptimal concentrations of Candida , Trichophyton-Oidiomyces-Epidermophyton and mumps virus was not enhanced in either group after 24 hours ' preculture apart from a slight increase in response to mumps virus in the patients .
	manualset3
160821	7	411808	7	NULL	NULL	0	NULL	24 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The production of migration inhibitory factor in response to suboptimal concentrations of Candida , Trichophyton-Oidiomyces-Epidermophyton and mumps virus was not enhanced in either group after 24 hours ' preculture apart from a slight increase in response to mumps virus in the patients .
	manualset3
160822	8	411808	7	NULL	NULL	0	NULL	preculture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The production of migration inhibitory factor in response to suboptimal concentrations of Candida , Trichophyton-Oidiomyces-Epidermophyton and mumps virus was not enhanced in either group after 24 hours ' preculture apart from a slight increase in response to mumps virus in the patients .
	manualset3
160823	9	411808	7	NULL	NULL	0	NULL	mumps virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The production of migration inhibitory factor in response to suboptimal concentrations of Candida , Trichophyton-Oidiomyces-Epidermophyton and mumps virus was not enhanced in either group after 24 hours ' preculture apart from a slight increase in response to mumps virus in the patients .
	manualset3
160824	10	411808	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The production of migration inhibitory factor in response to suboptimal concentrations of Candida , Trichophyton-Oidiomyces-Epidermophyton and mumps virus was not enhanced in either group after 24 hours ' preculture apart from a slight increase in response to mumps virus in the patients .
	manualset3
160825	1	411809	7	NULL	NULL	0	NULL	 profession	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The profession and the family ) .
	manualset3
160826	2	411809	7	NULL	NULL	0	NULL	family	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The profession and the family ) .
	manualset3
160827	1	411810	7	NULL	NULL	0	NULL	ATP-independent Ca2 + binding 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	ATP-independent Ca2 + binding , sialic acid and phospholipid content , Ca2 + ATPase , Mg2 + ATPase and adenylate-cyclase were not altered in membranes isolated by the hypotonic shock-LiBr treatment method from hypothyroid hearts .
	manualset3
160828	2	411810	7	NULL	NULL	0	NULL	sialic acid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	ATP-independent Ca2 + binding , sialic acid and phospholipid content , Ca2 + ATPase , Mg2 + ATPase and adenylate-cyclase were not altered in membranes isolated by the hypotonic shock-LiBr treatment method from hypothyroid hearts .
	manualset3
160829	3	411810	7	NULL	NULL	0	NULL	phospholipid content	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	ATP-independent Ca2 + binding , sialic acid and phospholipid content , Ca2 + ATPase , Mg2 + ATPase and adenylate-cyclase were not altered in membranes isolated by the hypotonic shock-LiBr treatment method from hypothyroid hearts .
	manualset3
160830	4	411810	7	NULL	NULL	0	NULL	Ca2 + ATPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	ATP-independent Ca2 + binding , sialic acid and phospholipid content , Ca2 + ATPase , Mg2 + ATPase and adenylate-cyclase were not altered in membranes isolated by the hypotonic shock-LiBr treatment method from hypothyroid hearts .
	manualset3
160831	5	411810	7	NULL	NULL	0	NULL	Mg2 + ATPase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	ATP-independent Ca2 + binding , sialic acid and phospholipid content , Ca2 + ATPase , Mg2 + ATPase and adenylate-cyclase were not altered in membranes isolated by the hypotonic shock-LiBr treatment method from hypothyroid hearts .
	manualset3
160832	6	411810	7	NULL	NULL	0	NULL	adenylate-cyclase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	ATP-independent Ca2 + binding , sialic acid and phospholipid content , Ca2 + ATPase , Mg2 + ATPase and adenylate-cyclase were not altered in membranes isolated by the hypotonic shock-LiBr treatment method from hypothyroid hearts .
	manualset3
160833	7	411810	7	NULL	NULL	0	NULL	membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	ATP-independent Ca2 + binding , sialic acid and phospholipid content , Ca2 + ATPase , Mg2 + ATPase and adenylate-cyclase were not altered in membranes isolated by the hypotonic shock-LiBr treatment method from hypothyroid hearts .
	manualset3
160834	8	411810	7	NULL	NULL	0	NULL	hypotonic shock-LiBr treatment method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	ATP-independent Ca2 + binding , sialic acid and phospholipid content , Ca2 + ATPase , Mg2 + ATPase and adenylate-cyclase were not altered in membranes isolated by the hypotonic shock-LiBr treatment method from hypothyroid hearts .
	manualset3
160835	9	411810	7	NULL	NULL	0	NULL	 hypothyroid hearts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	ATP-independent Ca2 + binding , sialic acid and phospholipid content , Ca2 + ATPase , Mg2 + ATPase and adenylate-cyclase were not altered in membranes isolated by the hypotonic shock-LiBr treatment method from hypothyroid hearts .
	manualset3
160836	1	411811	7	NULL	NULL	0	NULL	prognosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The prognosis of malignant tumors of the olfactory epithelium of the nasal vault stays very poor .
	manualset3
160837	2	411811	7	NULL	NULL	0	NULL	malignant tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prognosis of malignant tumors of the olfactory epithelium of the nasal vault stays very poor .
	manualset3
160838	3	411811	7	NULL	NULL	0	NULL	olfactory epithelium of the nasal vault 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The prognosis of malignant tumors of the olfactory epithelium of the nasal vault stays very poor .
	manualset3
160839	1	411812	7	NULL	NULL	0	NULL	prognosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prognosis of patients infected with human immunodeficiency virus ( HIV ) type 1 has dramatically improved since the advent of potent antiretroviral therapies ( ARTs ) , which have enabled sustained suppression of HIV replication and recovery of CD4 T cell counts .
	manualset3
160840	2	411812	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The prognosis of patients infected with human immunodeficiency virus ( HIV ) type 1 has dramatically improved since the advent of potent antiretroviral therapies ( ARTs ) , which have enabled sustained suppression of HIV replication and recovery of CD4 T cell counts .
	manualset3
160841	3	411812	7	NULL	NULL	0	NULL	human immunodeficiency virus ( HIV ) type 1	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The prognosis of patients infected with human immunodeficiency virus ( HIV ) type 1 has dramatically improved since the advent of potent antiretroviral therapies ( ARTs ) , which have enabled sustained suppression of HIV replication and recovery of CD4 T cell counts .
	manualset3
160842	4	411812	7	NULL	NULL	0	NULL	advent	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The prognosis of patients infected with human immunodeficiency virus ( HIV ) type 1 has dramatically improved since the advent of potent antiretroviral therapies ( ARTs ) , which have enabled sustained suppression of HIV replication and recovery of CD4 T cell counts .
	manualset3
160843	5	411812	7	NULL	NULL	0	NULL	 antiretroviral therapies ( ARTs )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The prognosis of patients infected with human immunodeficiency virus ( HIV ) type 1 has dramatically improved since the advent of potent antiretroviral therapies ( ARTs ) , which have enabled sustained suppression of HIV replication and recovery of CD4 T cell counts .
	manualset3
160844	6	411812	7	NULL	NULL	0	NULL	suppression 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The prognosis of patients infected with human immunodeficiency virus ( HIV ) type 1 has dramatically improved since the advent of potent antiretroviral therapies ( ARTs ) , which have enabled sustained suppression of HIV replication and recovery of CD4 T cell counts .
	manualset3
160845	7	411812	7	NULL	NULL	0	NULL	HIV replication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The prognosis of patients infected with human immunodeficiency virus ( HIV ) type 1 has dramatically improved since the advent of potent antiretroviral therapies ( ARTs ) , which have enabled sustained suppression of HIV replication and recovery of CD4 T cell counts .
	manualset3
160846	8	411812	7	NULL	NULL	0	NULL	recovery	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prognosis of patients infected with human immunodeficiency virus ( HIV ) type 1 has dramatically improved since the advent of potent antiretroviral therapies ( ARTs ) , which have enabled sustained suppression of HIV replication and recovery of CD4 T cell counts .
	manualset3
160847	9	411812	7	NULL	NULL	0	NULL	CD4 T cell counts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prognosis of patients infected with human immunodeficiency virus ( HIV ) type 1 has dramatically improved since the advent of potent antiretroviral therapies ( ARTs ) , which have enabled sustained suppression of HIV replication and recovery of CD4 T cell counts .
	manualset3
160848	1	411813	7	NULL	NULL	0	NULL	prognostic information 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The prognostic information provided by the cytosolic tPA : PAI-1 complex was comparable to that provided by cytosolic ( total ) PAI-1 .
	manualset3
160849	2	411813	7	NULL	NULL	0	NULL	 cytosolic tPA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The prognostic information provided by the cytosolic tPA : PAI-1 complex was comparable to that provided by cytosolic ( total ) PAI-1 .
	manualset3
160850	3	411813	7	NULL	NULL	0	NULL	PAI-1 complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The prognostic information provided by the cytosolic tPA : PAI-1 complex was comparable to that provided by cytosolic ( total ) PAI-1 .
	manualset3
160851	4	411813	7	NULL	NULL	0	NULL	cytosolic ( total ) PAI-1 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The prognostic information provided by the cytosolic tPA : PAI-1 complex was comparable to that provided by cytosolic ( total ) PAI-1 .
	manualset3
160852	1	411814	7	NULL	NULL	0	NULL	program	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The program requires at least one electrocardiogram with ST elevation of 200 microV or greater in the recording , caused by the current occlusion or by a previous occlusion , before it will yield a patency prediction .
	manualset3
160853	2	411814	7	NULL	NULL	NULL	NULL	 electrocardiogram	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The program requires at least one electrocardiogram with ST elevation of 200 microV or greater in the recording , caused by the current occlusion or by a previous occlusion , before it will yield a patency prediction .
	manualset3
160854	3	411814	7	NULL	NULL	0	NULL	ST elevation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The program requires at least one electrocardiogram with ST elevation of 200 microV or greater in the recording , caused by the current occlusion or by a previous occlusion , before it will yield a patency prediction .
	manualset3
160855	4	411814	7	NULL	NULL	0	NULL	200 microV	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The program requires at least one electrocardiogram with ST elevation of 200 microV or greater in the recording , caused by the current occlusion or by a previous occlusion , before it will yield a patency prediction .
	manualset3
160856	5	411814	7	NULL	NULL	0	NULL	recording	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The program requires at least one electrocardiogram with ST elevation of 200 microV or greater in the recording , caused by the current occlusion or by a previous occlusion , before it will yield a patency prediction .
	manualset3
160857	6	411814	7	NULL	NULL	0	NULL	current occlusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The program requires at least one electrocardiogram with ST elevation of 200 microV or greater in the recording , caused by the current occlusion or by a previous occlusion , before it will yield a patency prediction .
	manualset3
160858	7	411814	7	NULL	NULL	NULL	NULL	previous occlusion	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The program requires at least one electrocardiogram with ST elevation of 200 microV or greater in the recording , caused by the current occlusion or by a previous occlusion , before it will yield a patency prediction .
	manualset3
160859	8	411814	7	NULL	NULL	0	NULL	patency prediction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The program requires at least one electrocardiogram with ST elevation of 200 microV or greater in the recording , caused by the current occlusion or by a previous occlusion , before it will yield a patency prediction .
	manualset3
160860	1	411815	7	NULL	NULL	0	NULL	program	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The program was designed to teach school nurses in 7 rural counties in Maryland how to implement and to reinforce asthma management behaviors in children with asthma and their caregivers .
	manualset3
160861	2	411815	7	NULL	NULL	0	NULL	school nurses	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The program was designed to teach school nurses in 7 rural counties in Maryland how to implement and to reinforce asthma management behaviors in children with asthma and their caregivers .
	manualset3
160862	3	411815	7	NULL	NULL	0	NULL	7 rural counties	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The program was designed to teach school nurses in 7 rural counties in Maryland how to implement and to reinforce asthma management behaviors in children with asthma and their caregivers .
	manualset3
160863	4	411815	7	NULL	NULL	0	NULL	Maryland 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The program was designed to teach school nurses in 7 rural counties in Maryland how to implement and to reinforce asthma management behaviors in children with asthma and their caregivers .
	manualset3
160864	5	411815	7	NULL	NULL	0	NULL	asthma management behaviors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The program was designed to teach school nurses in 7 rural counties in Maryland how to implement and to reinforce asthma management behaviors in children with asthma and their caregivers .
	manualset3
160865	6	411815	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The program was designed to teach school nurses in 7 rural counties in Maryland how to implement and to reinforce asthma management behaviors in children with asthma and their caregivers .
	manualset3
160866	7	411815	7	NULL	NULL	0	NULL	asthma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The program was designed to teach school nurses in 7 rural counties in Maryland how to implement and to reinforce asthma management behaviors in children with asthma and their caregivers .
	manualset3
160867	8	411815	7	NULL	NULL	0	NULL	caregivers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The program was designed to teach school nurses in 7 rural counties in Maryland how to implement and to reinforce asthma management behaviors in children with asthma and their caregivers .
	manualset3
160868	1	411816	7	NULL	NULL	0	NULL	programmed component	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The programmed component of radiation response is significant in radiation oncology and predicted to create unique opportunities for enhanced treatment success .
	manualset3
160869	2	411816	7	NULL	NULL	0	NULL	radiation response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The programmed component of radiation response is significant in radiation oncology and predicted to create unique opportunities for enhanced treatment success .
	manualset3
160870	3	411816	7	NULL	NULL	0	NULL	radiation oncology	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The programmed component of radiation response is significant in radiation oncology and predicted to create unique opportunities for enhanced treatment success .
	manualset3
160871	4	411816	7	NULL	NULL	0	NULL	opportunities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The programmed component of radiation response is significant in radiation oncology and predicted to create unique opportunities for enhanced treatment success .
	manualset3
160872	5	411816	7	NULL	NULL	0	NULL	treatment success	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The programmed component of radiation response is significant in radiation oncology and predicted to create unique opportunities for enhanced treatment success .
	manualset3
160873	1	411817	7	NULL	NULL	0	NULL	project	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The project plans to provide for basic health needs through home visits by village health workers .
	manualset3
160875	2	411817	7	NULL	NULL	NULL	NULL	basic health needs	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The project plans to provide for basic health needs through home visits by village health workers .
	manualset3
160876	3	411817	7	NULL	NULL	NULL	NULL	home visits	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The project plans to provide for basic health needs through home visits by village health workers .
	manualset3
160877	4	411817	7	NULL	NULL	NULL	NULL	village health workers	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The project plans to provide for basic health needs through home visits by village health workers .
	manualset3
160878	1	411818	7	NULL	NULL	NULL	NULL	projection segmentation method	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The projection segmentation method , based on segmentation of high-attenuation features from the projections , effectively reduces artifacts caused by metal and large calcifications that can be reliably detected and segmented from projections .
	manualset3
160879	2	411818	7	NULL	NULL	0	NULL	segmentation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The projection segmentation method , based on segmentation of high-attenuation features from the projections , effectively reduces artifacts caused by metal and large calcifications that can be reliably detected and segmented from projections .
	manualset3
160880	3	411818	7	NULL	NULL	NULL	NULL	high-attenuation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The projection segmentation method , based on segmentation of high-attenuation features from the projections , effectively reduces artifacts caused by metal and large calcifications that can be reliably detected and segmented from projections .
	manualset3
160881	4	411818	7	NULL	NULL	NULL	NULL	 projections	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The projection segmentation method , based on segmentation of high-attenuation features from the projections , effectively reduces artifacts caused by metal and large calcifications that can be reliably detected and segmented from projections .
	manualset3
160882	5	411818	7	NULL	NULL	0	NULL	artifacts	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The projection segmentation method , based on segmentation of high-attenuation features from the projections , effectively reduces artifacts caused by metal and large calcifications that can be reliably detected and segmented from projections .
	manualset3
160883	6	411818	7	NULL	NULL	0	NULL	metal 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The projection segmentation method , based on segmentation of high-attenuation features from the projections , effectively reduces artifacts caused by metal and large calcifications that can be reliably detected and segmented from projections .
	manualset3
160884	7	411818	7	NULL	NULL	NULL	NULL	large calcifications	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The projection segmentation method , based on segmentation of high-attenuation features from the projections , effectively reduces artifacts caused by metal and large calcifications that can be reliably detected and segmented from projections .
	manualset3
160885	8	411818	7	NULL	NULL	NULL	NULL	projections	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The projection segmentation method , based on segmentation of high-attenuation features from the projections , effectively reduces artifacts caused by metal and large calcifications that can be reliably detected and segmented from projections .
	manualset3
160886	1	411819	7	NULL	NULL	0	NULL	Clinical study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical study of total plasma volume , total body exchangeable sodium and plasma renin activity in patients with maintenance hemodialysis ( author 's transl ) ) .
	manualset3
160887	2	411819	7	NULL	NULL	0	NULL	total plasma volume	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical study of total plasma volume , total body exchangeable sodium and plasma renin activity in patients with maintenance hemodialysis ( author 's transl ) ) .
	manualset3
160888	3	411819	7	NULL	NULL	0	NULL	 total body exchangeable sodium activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical study of total plasma volume , total body exchangeable sodium and plasma renin activity in patients with maintenance hemodialysis ( author 's transl ) ) .
	manualset3
160889	4	411819	7	NULL	NULL	0	NULL	plasma renin activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical study of total plasma volume , total body exchangeable sodium and plasma renin activity in patients with maintenance hemodialysis ( author 's transl ) ) .
	manualset3
160890	5	411819	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical study of total plasma volume , total body exchangeable sodium and plasma renin activity in patients with maintenance hemodialysis ( author 's transl ) ) .
	manualset3
160891	6	411819	7	NULL	NULL	0	NULL	hemodialysis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical study of total plasma volume , total body exchangeable sodium and plasma renin activity in patients with maintenance hemodialysis ( author 's transl ) ) .
	manualset3
160892	7	411819	7	NULL	NULL	0	NULL	author 's transl	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical study of total plasma volume , total body exchangeable sodium and plasma renin activity in patients with maintenance hemodialysis ( author 's transl ) ) .
	manualset3
160893	1	411820	7	NULL	NULL	0	NULL	ATP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	ATP , acting through P2X ( 2 ) / P2X ( 3 ) receptor-channel complexes , plays an important role in carotid body chemoexcitation in response to natural stimuli in the rat .
	manualset3
160894	2	411820	7	NULL	NULL	0	NULL	 P2X ( 2 ) / P2X ( 3 ) receptor-channel complexes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	ATP , acting through P2X ( 2 ) / P2X ( 3 ) receptor-channel complexes , plays an important role in carotid body chemoexcitation in response to natural stimuli in the rat .
	manualset3
160895	3	411820	7	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	ATP , acting through P2X ( 2 ) / P2X ( 3 ) receptor-channel complexes , plays an important role in carotid body chemoexcitation in response to natural stimuli in the rat .
	manualset3
160896	4	411820	7	NULL	NULL	0	NULL	carotid body chemoexcitation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	ATP , acting through P2X ( 2 ) / P2X ( 3 ) receptor-channel complexes , plays an important role in carotid body chemoexcitation in response to natural stimuli in the rat .
	manualset3
160897	5	411820	7	NULL	NULL	0	NULL	natural stimuli	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	ATP , acting through P2X ( 2 ) / P2X ( 3 ) receptor-channel complexes , plays an important role in carotid body chemoexcitation in response to natural stimuli in the rat .
	manualset3
160898	6	411820	7	NULL	NULL	0	NULL	rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	ATP , acting through P2X ( 2 ) / P2X ( 3 ) receptor-channel complexes , plays an important role in carotid body chemoexcitation in response to natural stimuli in the rat .
	manualset3
169340	7	411820	7	NULL	NULL	0	NULL	 response	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	ATP , acting through P2X ( 2 ) / P2X ( 3 ) receptor-channel complexes , plays an important role in carotid body chemoexcitation in response to natural stimuli in the rat .
	manualset3
160899	1	411821	7	NULL	NULL	0	NULL	 proliferating cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The proliferating cells were S100 , CD1a and CD207 ( langerin ) positive and cytokeratin , epithelial membrane antigen , CD15 , CD30 , melan A and carcinoembryonic antigen negative .
	manualset3
160900	2	411821	7	NULL	NULL	0	NULL	S100	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proliferating cells were S100 , CD1a and CD207 ( langerin ) positive and cytokeratin , epithelial membrane antigen , CD15 , CD30 , melan A and carcinoembryonic antigen negative .
	manualset3
160901	3	411821	7	NULL	NULL	0	NULL	CD1a 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proliferating cells were S100 , CD1a and CD207 ( langerin ) positive and cytokeratin , epithelial membrane antigen , CD15 , CD30 , melan A and carcinoembryonic antigen negative .
	manualset3
160902	4	411821	7	NULL	NULL	0	NULL	CD207 ( langerin ) positive	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proliferating cells were S100 , CD1a and CD207 ( langerin ) positive and cytokeratin , epithelial membrane antigen , CD15 , CD30 , melan A and carcinoembryonic antigen negative .
	manualset3
160903	5	411821	7	NULL	NULL	0	NULL	cytokeratin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proliferating cells were S100 , CD1a and CD207 ( langerin ) positive and cytokeratin , epithelial membrane antigen , CD15 , CD30 , melan A and carcinoembryonic antigen negative .
	manualset3
160904	6	411821	7	NULL	NULL	0	NULL	epithelial membrane antigen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proliferating cells were S100 , CD1a and CD207 ( langerin ) positive and cytokeratin , epithelial membrane antigen , CD15 , CD30 , melan A and carcinoembryonic antigen negative .
	manualset3
160905	7	411821	7	NULL	NULL	0	NULL	CD15	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proliferating cells were S100 , CD1a and CD207 ( langerin ) positive and cytokeratin , epithelial membrane antigen , CD15 , CD30 , melan A and carcinoembryonic antigen negative .
	manualset3
160906	8	411821	7	NULL	NULL	0	NULL	CD30 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proliferating cells were S100 , CD1a and CD207 ( langerin ) positive and cytokeratin , epithelial membrane antigen , CD15 , CD30 , melan A and carcinoembryonic antigen negative .
	manualset3
160907	9	411821	7	NULL	NULL	0	NULL	melan A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proliferating cells were S100 , CD1a and CD207 ( langerin ) positive and cytokeratin , epithelial membrane antigen , CD15 , CD30 , melan A and carcinoembryonic antigen negative .
	manualset3
160908	10	411821	7	NULL	NULL	0	NULL	carcinoembryonic antigen negative	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proliferating cells were S100 , CD1a and CD207 ( langerin ) positive and cytokeratin , epithelial membrane antigen , CD15 , CD30 , melan A and carcinoembryonic antigen negative .
	manualset3
160909	1	411822	7	NULL	NULL	0	NULL	proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The proliferation of megakaryocyte progenitors was also stimulated by partially purified interleukin 3 , whereas both human recombinant erythropoietin and human recombinant granulocyte colony-stimulating factor ( rG-CSF ) failed to modify the incorporation of serotonin in comparison with unstimulated cultures .
	manualset3
160910	2	411822	7	NULL	NULL	0	NULL	megakaryocyte progenitors	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The proliferation of megakaryocyte progenitors was also stimulated by partially purified interleukin 3 , whereas both human recombinant erythropoietin and human recombinant granulocyte colony-stimulating factor ( rG-CSF ) failed to modify the incorporation of serotonin in comparison with unstimulated cultures .
	manualset3
160911	3	411822	7	NULL	NULL	0	NULL	purified interleukin 3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proliferation of megakaryocyte progenitors was also stimulated by partially purified interleukin 3 , whereas both human recombinant erythropoietin and human recombinant granulocyte colony-stimulating factor ( rG-CSF ) failed to modify the incorporation of serotonin in comparison with unstimulated cultures .
	manualset3
160912	4	411822	7	NULL	NULL	0	NULL	human recombinant erythropoietin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proliferation of megakaryocyte progenitors was also stimulated by partially purified interleukin 3 , whereas both human recombinant erythropoietin and human recombinant granulocyte colony-stimulating factor ( rG-CSF ) failed to modify the incorporation of serotonin in comparison with unstimulated cultures .
	manualset3
160913	5	411822	7	NULL	NULL	0	NULL	human recombinant granulocyte colony-stimulating factor ( rG-CSF )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proliferation of megakaryocyte progenitors was also stimulated by partially purified interleukin 3 , whereas both human recombinant erythropoietin and human recombinant granulocyte colony-stimulating factor ( rG-CSF ) failed to modify the incorporation of serotonin in comparison with unstimulated cultures .
	manualset3
160914	6	411822	7	NULL	NULL	0	NULL	 incorporation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The proliferation of megakaryocyte progenitors was also stimulated by partially purified interleukin 3 , whereas both human recombinant erythropoietin and human recombinant granulocyte colony-stimulating factor ( rG-CSF ) failed to modify the incorporation of serotonin in comparison with unstimulated cultures .
	manualset3
160915	7	411822	7	NULL	NULL	0	NULL	serotonin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The proliferation of megakaryocyte progenitors was also stimulated by partially purified interleukin 3 , whereas both human recombinant erythropoietin and human recombinant granulocyte colony-stimulating factor ( rG-CSF ) failed to modify the incorporation of serotonin in comparison with unstimulated cultures .
	manualset3
160916	8	411822	7	NULL	NULL	0	NULL	unstimulated cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The proliferation of megakaryocyte progenitors was also stimulated by partially purified interleukin 3 , whereas both human recombinant erythropoietin and human recombinant granulocyte colony-stimulating factor ( rG-CSF ) failed to modify the incorporation of serotonin in comparison with unstimulated cultures .
	manualset3
160917	1	411823	7	NULL	NULL	0	NULL	proliferative capacity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The proliferative capacity and morphology of hCECs are vastly affected by the four culture media .
	manualset3
160918	2	411823	7	NULL	NULL	0	NULL	morphology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proliferative capacity and morphology of hCECs are vastly affected by the four culture media .
	manualset3
160919	3	411823	7	NULL	NULL	0	NULL	hCECs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The proliferative capacity and morphology of hCECs are vastly affected by the four culture media .
	manualset3
160920	4	411823	7	NULL	NULL	NULL	NULL	four culture media	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proliferative capacity and morphology of hCECs are vastly affected by the four culture media .
	manualset3
160921	1	411824	7	NULL	NULL	0	NULL	promoter activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The promoter activity of Rab4 was increased by metformin in an AMPK-dependent manner .
	manualset3
160922	2	411824	7	NULL	NULL	0	NULL	Rab4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The promoter activity of Rab4 was increased by metformin in an AMPK-dependent manner .
	manualset3
160923	3	411824	7	NULL	NULL	0	NULL	metformin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The promoter activity of Rab4 was increased by metformin in an AMPK-dependent manner .
	manualset3
160924	4	411824	7	NULL	NULL	0	NULL	AMPK-dependent manner	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The promoter activity of Rab4 was increased by metformin in an AMPK-dependent manner .
	manualset3
160925	1	411825	7	NULL	NULL	0	NULL	 promoter activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The promoter activity was monitored during the differentiation of this cell line elicited by the sequential treatment with retinoic acid and brain-derived neurotrophic factor ( BDNF ) .
	manualset3
160926	2	411825	7	NULL	NULL	0	NULL	differentiation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The promoter activity was monitored during the differentiation of this cell line elicited by the sequential treatment with retinoic acid and brain-derived neurotrophic factor ( BDNF ) .
	manualset3
160927	3	411825	7	NULL	NULL	0	NULL	cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The promoter activity was monitored during the differentiation of this cell line elicited by the sequential treatment with retinoic acid and brain-derived neurotrophic factor ( BDNF ) .
	manualset3
160928	4	411825	7	NULL	NULL	0	NULL	treatment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The promoter activity was monitored during the differentiation of this cell line elicited by the sequential treatment with retinoic acid and brain-derived neurotrophic factor ( BDNF ) .
	manualset3
160929	5	411825	7	NULL	NULL	0	NULL	retinoic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The promoter activity was monitored during the differentiation of this cell line elicited by the sequential treatment with retinoic acid and brain-derived neurotrophic factor ( BDNF ) .
	manualset3
160930	6	411825	7	NULL	NULL	0	NULL	brain-derived neurotrophic factor ( BDNF )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The promoter activity was monitored during the differentiation of this cell line elicited by the sequential treatment with retinoic acid and brain-derived neurotrophic factor ( BDNF ) .
	manualset3
160932	1	411826	7	NULL	NULL	NULL	NULL	promoter of filamentation ( POF1 ) protein	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The promoter of filamentation ( POF1 ) protein from Saccharomyces cerevisiae is an ATPase involved in the protein quality control process .
	manualset3
160933	2	411826	7	NULL	NULL	NULL	NULL	Saccharomyces cerevisiae	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The promoter of filamentation ( POF1 ) protein from Saccharomyces cerevisiae is an ATPase involved in the protein quality control process .
	manualset3
160934	3	411826	7	NULL	NULL	NULL	NULL	 ATPase	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The promoter of filamentation ( POF1 ) protein from Saccharomyces cerevisiae is an ATPase involved in the protein quality control process .
	manualset3
160935	4	411826	7	NULL	NULL	NULL	NULL	protein quality control process	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The promoter of filamentation ( POF1 ) protein from Saccharomyces cerevisiae is an ATPase involved in the protein quality control process .
	manualset3
160936	1	411827	7	NULL	NULL	0	NULL	promoters 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The promoters of these genes contain a putative HY5 binding site , and in line with this observation , HY5 can bind to the promoter of AXR2 in vitro .
	manualset3
160937	2	411827	7	NULL	NULL	0	NULL	genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The promoters of these genes contain a putative HY5 binding site , and in line with this observation , HY5 can bind to the promoter of AXR2 in vitro .
	manualset3
160938	3	411827	7	NULL	NULL	NULL	NULL	putative HY5 binding site	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The promoters of these genes contain a putative HY5 binding site , and in line with this observation , HY5 can bind to the promoter of AXR2 in vitro .
	manualset3
160939	4	411827	7	NULL	NULL	0	NULL	HY5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The promoters of these genes contain a putative HY5 binding site , and in line with this observation , HY5 can bind to the promoter of AXR2 in vitro .
	manualset3
160940	5	411827	7	NULL	NULL	0	NULL	promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The promoters of these genes contain a putative HY5 binding site , and in line with this observation , HY5 can bind to the promoter of AXR2 in vitro .
	manualset3
160941	6	411827	7	NULL	NULL	0	NULL	AXR2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The promoters of these genes contain a putative HY5 binding site , and in line with this observation , HY5 can bind to the promoter of AXR2 in vitro .
	manualset3
169341	7	411827	7	NULL	NULL	0	NULL	observation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The promoters of these genes contain a putative HY5 binding site , and in line with this observation , HY5 can bind to the promoter of AXR2 in vitro .
	manualset3
160942	1	411828	7	NULL	NULL	0	NULL	promyelocytic leukemia gene PML	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The promyelocytic leukemia gene PML was originally identified at the t ( 15 ; 17 ) translocation of acute promyelocytic leukemia , which generates the oncogene PML-retinoic acid receptor .
	manualset3
160943	2	411828	7	NULL	NULL	0	NULL	t ( 15 ; 17 ) translocation	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The promyelocytic leukemia gene PML was originally identified at the t ( 15 ; 17 ) translocation of acute promyelocytic leukemia , which generates the oncogene PML-retinoic acid receptor .
	manualset3
160944	3	411828	7	NULL	NULL	0	NULL	acute promyelocytic leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The promyelocytic leukemia gene PML was originally identified at the t ( 15 ; 17 ) translocation of acute promyelocytic leukemia , which generates the oncogene PML-retinoic acid receptor .
	manualset3
160945	4	411828	7	NULL	NULL	0	NULL	oncogene PML-retinoic acid receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The promyelocytic leukemia gene PML was originally identified at the t ( 15 ; 17 ) translocation of acute promyelocytic leukemia , which generates the oncogene PML-retinoic acid receptor .
	manualset3
160946	1	411829	7	NULL	NULL	NULL	NULL	 management 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proper management is not only rewarding in terms of responsiveness in an otherwise `` incurable '' and progressive disease , but also improves the quality of life of the patients and the caregivers alike .
	manualset3
160947	2	411829	7	NULL	NULL	0	NULL	incurable	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The proper management is not only rewarding in terms of responsiveness in an otherwise `` incurable '' and progressive disease , but also improves the quality of life of the patients and the caregivers alike .
	manualset3
160948	3	411829	7	NULL	NULL	0	NULL	progressive disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The proper management is not only rewarding in terms of responsiveness in an otherwise `` incurable '' and progressive disease , but also improves the quality of life of the patients and the caregivers alike .
	manualset3
160949	4	411829	7	NULL	NULL	NULL	NULL	quality	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proper management is not only rewarding in terms of responsiveness in an otherwise `` incurable '' and progressive disease , but also improves the quality of life of the patients and the caregivers alike .
	manualset3
160950	5	411829	7	NULL	NULL	0	NULL	life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The proper management is not only rewarding in terms of responsiveness in an otherwise `` incurable '' and progressive disease , but also improves the quality of life of the patients and the caregivers alike .
	manualset3
160951	6	411829	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The proper management is not only rewarding in terms of responsiveness in an otherwise `` incurable '' and progressive disease , but also improves the quality of life of the patients and the caregivers alike .
	manualset3
160952	7	411829	7	NULL	NULL	0	NULL	caregivers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The proper management is not only rewarding in terms of responsiveness in an otherwise `` incurable '' and progressive disease , but also improves the quality of life of the patients and the caregivers alike .
	manualset3
169342	8	411829	7	NULL	NULL	0	NULL	terms	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proper management is not only rewarding in terms of responsiveness in an otherwise `` incurable '' and progressive disease , but also improves the quality of life of the patients and the caregivers alike .
	manualset3
169343	9	411829	7	NULL	NULL	0	NULL	 responsiveness	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proper management is not only rewarding in terms of responsiveness in an otherwise `` incurable '' and progressive disease , but also improves the quality of life of the patients and the caregivers alike .
	manualset3
160953	1	411830	7	NULL	NULL	0	NULL	Bpu XynA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The properties Bpu XynA make it promising for application in the production of Bifidobacterium growth-promoting factors and in feed industry .
	manualset3
160954	2	411830	7	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The properties Bpu XynA make it promising for application in the production of Bifidobacterium growth-promoting factors and in feed industry .
	manualset3
160955	3	411830	7	NULL	NULL	0	NULL	production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The properties Bpu XynA make it promising for application in the production of Bifidobacterium growth-promoting factors and in feed industry .
	manualset3
160956	4	411830	7	NULL	NULL	0	NULL	Bifidobacterium	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The properties Bpu XynA make it promising for application in the production of Bifidobacterium growth-promoting factors and in feed industry .
	manualset3
160957	5	411830	7	NULL	NULL	0	NULL	growth-promoting factors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The properties Bpu XynA make it promising for application in the production of Bifidobacterium growth-promoting factors and in feed industry .
	manualset3
160958	6	411830	7	NULL	NULL	0	NULL	feed industry	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The properties Bpu XynA make it promising for application in the production of Bifidobacterium growth-promoting factors and in feed industry .
	manualset3
160964	1	411831	7	NULL	NULL	0	NULL	properties	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The properties of H ( + ) - ATPase from rat liver lysosomes were analyzed by reconstituting proton pump activity from solubilized enzyme and Escherichia coli phospholipids in proteoliposomes devoid of anion-channels .
	manualset3
160965	2	411831	7	NULL	NULL	0	NULL	H ( + ) - ATPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The properties of H ( + ) - ATPase from rat liver lysosomes were analyzed by reconstituting proton pump activity from solubilized enzyme and Escherichia coli phospholipids in proteoliposomes devoid of anion-channels .
	manualset3
160966	3	411831	7	NULL	NULL	0	NULL	 rat liver lysosomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The properties of H ( + ) - ATPase from rat liver lysosomes were analyzed by reconstituting proton pump activity from solubilized enzyme and Escherichia coli phospholipids in proteoliposomes devoid of anion-channels .
	manualset3
160967	4	411831	7	NULL	NULL	0	NULL	proton pump activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The properties of H ( + ) - ATPase from rat liver lysosomes were analyzed by reconstituting proton pump activity from solubilized enzyme and Escherichia coli phospholipids in proteoliposomes devoid of anion-channels .
	manualset3
160968	5	411831	7	NULL	NULL	0	NULL	 solubilized enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The properties of H ( + ) - ATPase from rat liver lysosomes were analyzed by reconstituting proton pump activity from solubilized enzyme and Escherichia coli phospholipids in proteoliposomes devoid of anion-channels .
	manualset3
160969	6	411831	7	NULL	NULL	0	NULL	Escherichia coli phospholipids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The properties of H ( + ) - ATPase from rat liver lysosomes were analyzed by reconstituting proton pump activity from solubilized enzyme and Escherichia coli phospholipids in proteoliposomes devoid of anion-channels .
	manualset3
160970	7	411831	7	NULL	NULL	NULL	NULL	proteoliposomes	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The properties of H ( + ) - ATPase from rat liver lysosomes were analyzed by reconstituting proton pump activity from solubilized enzyme and Escherichia coli phospholipids in proteoliposomes devoid of anion-channels .
	manualset3
160971	8	411831	7	NULL	NULL	0	NULL	anion-channels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The properties of H ( + ) - ATPase from rat liver lysosomes were analyzed by reconstituting proton pump activity from solubilized enzyme and Escherichia coli phospholipids in proteoliposomes devoid of anion-channels .
	manualset3
160972	1	411832	7	NULL	NULL	0	NULL	properties	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The properties of iodine in solutions of surface-active agents .
	manualset3
160973	2	411832	7	NULL	NULL	0	NULL	 iodine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The properties of iodine in solutions of surface-active agents .
	manualset3
160974	3	411832	7	NULL	NULL	0	NULL	solutions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The properties of iodine in solutions of surface-active agents .
	manualset3
160975	4	411832	7	NULL	NULL	0	NULL	surface-active agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The properties of iodine in solutions of surface-active agents .
	manualset3
160976	1	411833	7	NULL	NULL	NULL	NULL	 proportion	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proportion ` cured ' is defined as the proportion of survivors for whom , as a group , there is no longer excess mortality compared to the general population .
	manualset3
160978	3	411833	7	NULL	NULL	NULL	NULL	 proportion	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proportion ` cured ' is defined as the proportion of survivors for whom , as a group , there is no longer excess mortality compared to the general population .
	manualset3
160979	4	411833	7	NULL	NULL	0	NULL	group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion ` cured ' is defined as the proportion of survivors for whom , as a group , there is no longer excess mortality compared to the general population .
	manualset3
160980	5	411833	7	NULL	NULL	NULL	NULL	mortality	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proportion ` cured ' is defined as the proportion of survivors for whom , as a group , there is no longer excess mortality compared to the general population .
	manualset3
160981	6	411833	7	NULL	NULL	0	NULL	general population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion ` cured ' is defined as the proportion of survivors for whom , as a group , there is no longer excess mortality compared to the general population .
	manualset3
162351	7	411833	7	NULL	NULL	0	NULL	survivors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion ` cured ' is defined as the proportion of survivors for whom , as a group , there is no longer excess mortality compared to the general population .
	manualset3
160982	1	411834	7	NULL	NULL	0	NULL	 proportion 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of 121Q carriers progressively increased in the three groups ( 27.4 , 28.8 , and 33.2 % , respectively ; adjusted P value = 0.027 ) .
	manualset3
160983	2	411834	7	NULL	NULL	0	NULL	121Q carriers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of 121Q carriers progressively increased in the three groups ( 27.4 , 28.8 , and 33.2 % , respectively ; adjusted P value = 0.027 ) .
	manualset3
160984	3	411834	7	NULL	NULL	0	NULL	three groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of 121Q carriers progressively increased in the three groups ( 27.4 , 28.8 , and 33.2 % , respectively ; adjusted P value = 0.027 ) .
	manualset3
160985	4	411834	7	NULL	NULL	0	NULL	27.4 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of 121Q carriers progressively increased in the three groups ( 27.4 , 28.8 , and 33.2 % , respectively ; adjusted P value = 0.027 ) .
	manualset3
160986	5	411834	7	NULL	NULL	0	NULL	28.8%	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of 121Q carriers progressively increased in the three groups ( 27.4 , 28.8 , and 33.2 % , respectively ; adjusted P value = 0.027 ) .
	manualset3
160987	6	411834	7	NULL	NULL	0	NULL	33.2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of 121Q carriers progressively increased in the three groups ( 27.4 , 28.8 , and 33.2 % , respectively ; adjusted P value = 0.027 ) .
	manualset3
160988	7	411834	7	NULL	NULL	0	NULL	P value = 0.027	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of 121Q carriers progressively increased in the three groups ( 27.4 , 28.8 , and 33.2 % , respectively ; adjusted P value = 0.027 ) .
	manualset3
160989	1	411835	7	NULL	NULL	NULL	NULL	proportion 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proportion of fat in the diets of the overweight and obese women irrespective of PCOS was well-above current recommendations , yet this excessive fat intake occurred at the expense of monounsaturated fatty acids mostly .
	manualset3
160990	2	411835	7	NULL	NULL	0	NULL	diets 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of fat in the diets of the overweight and obese women irrespective of PCOS was well-above current recommendations , yet this excessive fat intake occurred at the expense of monounsaturated fatty acids mostly .
	manualset3
160991	3	411835	7	NULL	NULL	0	NULL	overweight and obese women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of fat in the diets of the overweight and obese women irrespective of PCOS was well-above current recommendations , yet this excessive fat intake occurred at the expense of monounsaturated fatty acids mostly .
	manualset3
160992	4	411835	7	NULL	NULL	0	NULL	PCOS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of fat in the diets of the overweight and obese women irrespective of PCOS was well-above current recommendations , yet this excessive fat intake occurred at the expense of monounsaturated fatty acids mostly .
	manualset3
160993	5	411835	7	NULL	NULL	0	NULL	 recommendations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of fat in the diets of the overweight and obese women irrespective of PCOS was well-above current recommendations , yet this excessive fat intake occurred at the expense of monounsaturated fatty acids mostly .
	manualset3
160994	6	411835	7	NULL	NULL	NULL	NULL	fat intake	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proportion of fat in the diets of the overweight and obese women irrespective of PCOS was well-above current recommendations , yet this excessive fat intake occurred at the expense of monounsaturated fatty acids mostly .
	manualset3
160995	7	411835	7	NULL	NULL	0	NULL	expense	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of fat in the diets of the overweight and obese women irrespective of PCOS was well-above current recommendations , yet this excessive fat intake occurred at the expense of monounsaturated fatty acids mostly .
	manualset3
160996	8	411835	7	NULL	NULL	0	NULL	monounsaturated fatty acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of fat in the diets of the overweight and obese women irrespective of PCOS was well-above current recommendations , yet this excessive fat intake occurred at the expense of monounsaturated fatty acids mostly .
	manualset3
162352	9	411835	7	NULL	NULL	0	NULL	fat	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of fat in the diets of the overweight and obese women irrespective of PCOS was well-above current recommendations , yet this excessive fat intake occurred at the expense of monounsaturated fatty acids mostly .
	manualset3
160997	1	411836	7	NULL	NULL	0	NULL	AVP stimulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	AVP stimulation of myoblasts induced the rapid formation of stress fiber-like actin structures ( SFLSs ) .
	manualset3
160998	2	411836	7	NULL	NULL	0	NULL	myoblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	AVP stimulation of myoblasts induced the rapid formation of stress fiber-like actin structures ( SFLSs ) .
	manualset3
160999	3	411836	7	NULL	NULL	0	NULL	formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	AVP stimulation of myoblasts induced the rapid formation of stress fiber-like actin structures ( SFLSs ) .
	manualset3
161000	4	411836	7	NULL	NULL	0	NULL	stress fiber-like actin structures ( SFLSs )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	AVP stimulation of myoblasts induced the rapid formation of stress fiber-like actin structures ( SFLSs ) .
	manualset3
161008	1	411837	7	NULL	NULL	NULL	NULL	proportion	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proportion of illiterates among the tubectomy acceptors was 67.4 % in Group A and 61.7 % in Groups B and C. Acceptance of tubectomy among the agricultural laborers increased from 21.9 % in Group A to 30.9 % in Group C , showing an overall increase of 9 % over the years .
	manualset3
161009	2	411837	7	NULL	NULL	0	NULL	tubectomy acceptors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of illiterates among the tubectomy acceptors was 67.4 % in Group A and 61.7 % in Groups B and C. Acceptance of tubectomy among the agricultural laborers increased from 21.9 % in Group A to 30.9 % in Group C , showing an overall increase of 9 % over the years .
	manualset3
161010	3	411837	7	NULL	NULL	0	NULL	67.4 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of illiterates among the tubectomy acceptors was 67.4 % in Group A and 61.7 % in Groups B and C. Acceptance of tubectomy among the agricultural laborers increased from 21.9 % in Group A to 30.9 % in Group C , showing an overall increase of 9 % over the years .
	manualset3
161011	4	411837	7	NULL	NULL	0	NULL	Group A	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of illiterates among the tubectomy acceptors was 67.4 % in Group A and 61.7 % in Groups B and C. Acceptance of tubectomy among the agricultural laborers increased from 21.9 % in Group A to 30.9 % in Group C , showing an overall increase of 9 % over the years .
	manualset3
161012	5	411837	7	NULL	NULL	NULL	NULL	61.7 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proportion of illiterates among the tubectomy acceptors was 67.4 % in Group A and 61.7 % in Groups B and C. Acceptance of tubectomy among the agricultural laborers increased from 21.9 % in Group A to 30.9 % in Group C , showing an overall increase of 9 % over the years .
	manualset3
161013	6	411837	7	NULL	NULL	0	NULL	Groups B	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of illiterates among the tubectomy acceptors was 67.4 % in Group A and 61.7 % in Groups B and C. Acceptance of tubectomy among the agricultural laborers increased from 21.9 % in Group A to 30.9 % in Group C , showing an overall increase of 9 % over the years .
	manualset3
161014	7	411837	7	NULL	NULL	0	NULL	Groups C	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of illiterates among the tubectomy acceptors was 67.4 % in Group A and 61.7 % in Groups B and C. Acceptance of tubectomy among the agricultural laborers increased from 21.9 % in Group A to 30.9 % in Group C , showing an overall increase of 9 % over the years .
	manualset3
161015	8	411837	7	NULL	NULL	0	NULL	tubectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of illiterates among the tubectomy acceptors was 67.4 % in Group A and 61.7 % in Groups B and C. Acceptance of tubectomy among the agricultural laborers increased from 21.9 % in Group A to 30.9 % in Group C , showing an overall increase of 9 % over the years .
	manualset3
161016	9	411837	7	NULL	NULL	0	NULL	agricultural laborers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of illiterates among the tubectomy acceptors was 67.4 % in Group A and 61.7 % in Groups B and C. Acceptance of tubectomy among the agricultural laborers increased from 21.9 % in Group A to 30.9 % in Group C , showing an overall increase of 9 % over the years .
	manualset3
161017	10	411837	7	NULL	NULL	0	NULL	21.9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of illiterates among the tubectomy acceptors was 67.4 % in Group A and 61.7 % in Groups B and C. Acceptance of tubectomy among the agricultural laborers increased from 21.9 % in Group A to 30.9 % in Group C , showing an overall increase of 9 % over the years .
	manualset3
161018	11	411837	7	NULL	NULL	0	NULL	Group A	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of illiterates among the tubectomy acceptors was 67.4 % in Group A and 61.7 % in Groups B and C. Acceptance of tubectomy among the agricultural laborers increased from 21.9 % in Group A to 30.9 % in Group C , showing an overall increase of 9 % over the years .
	manualset3
161019	12	411837	7	NULL	NULL	0	NULL	30.9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of illiterates among the tubectomy acceptors was 67.4 % in Group A and 61.7 % in Groups B and C. Acceptance of tubectomy among the agricultural laborers increased from 21.9 % in Group A to 30.9 % in Group C , showing an overall increase of 9 % over the years .
	manualset3
161020	13	411837	7	NULL	NULL	0	NULL	Group C	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of illiterates among the tubectomy acceptors was 67.4 % in Group A and 61.7 % in Groups B and C. Acceptance of tubectomy among the agricultural laborers increased from 21.9 % in Group A to 30.9 % in Group C , showing an overall increase of 9 % over the years .
	manualset3
161021	14	411837	7	NULL	NULL	0	NULL	 9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of illiterates among the tubectomy acceptors was 67.4 % in Group A and 61.7 % in Groups B and C. Acceptance of tubectomy among the agricultural laborers increased from 21.9 % in Group A to 30.9 % in Group C , showing an overall increase of 9 % over the years .
	manualset3
161022	15	411837	7	NULL	NULL	0	NULL	years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of illiterates among the tubectomy acceptors was 67.4 % in Group A and 61.7 % in Groups B and C. Acceptance of tubectomy among the agricultural laborers increased from 21.9 % in Group A to 30.9 % in Group C , showing an overall increase of 9 % over the years .
	manualset3
162353	16	411837	7	NULL	NULL	0	NULL	 illiterates	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of illiterates among the tubectomy acceptors was 67.4 % in Group A and 61.7 % in Groups B and C. Acceptance of tubectomy among the agricultural laborers increased from 21.9 % in Group A to 30.9 % in Group C , showing an overall increase of 9 % over the years .
	manualset3
161023	1	411838	7	NULL	NULL	0	NULL	proportion	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of natural pesticides positive in animal tests of clastogenicity is also the same as for synthetic chemicals .
	manualset3
161024	2	411838	7	NULL	NULL	0	NULL	natural pesticides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of natural pesticides positive in animal tests of clastogenicity is also the same as for synthetic chemicals .
	manualset3
161025	3	411838	7	NULL	NULL	0	NULL	animal tests 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of natural pesticides positive in animal tests of clastogenicity is also the same as for synthetic chemicals .
	manualset3
161026	4	411838	7	NULL	NULL	0	NULL	clastogenicity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of natural pesticides positive in animal tests of clastogenicity is also the same as for synthetic chemicals .
	manualset3
161027	5	411838	7	NULL	NULL	0	NULL	synthetic chemicals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of natural pesticides positive in animal tests of clastogenicity is also the same as for synthetic chemicals .
	manualset3
161028	1	411839	7	NULL	NULL	0	NULL	 proportion	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of occupational skin diseases in relation to all occupational diseases has gradually decreased from 51.7 % in 1973 to 16.3 % in 1998 , in absolute figures from 382 cases in 1973 decreased to 60 cases in 1998 .
	manualset3
161029	2	411839	7	NULL	NULL	0	NULL	occupational skin diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of occupational skin diseases in relation to all occupational diseases has gradually decreased from 51.7 % in 1973 to 16.3 % in 1998 , in absolute figures from 382 cases in 1973 decreased to 60 cases in 1998 .
	manualset3
161030	3	411839	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of occupational skin diseases in relation to all occupational diseases has gradually decreased from 51.7 % in 1973 to 16.3 % in 1998 , in absolute figures from 382 cases in 1973 decreased to 60 cases in 1998 .
	manualset3
161031	4	411839	7	NULL	NULL	0	NULL	occupational diseases 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of occupational skin diseases in relation to all occupational diseases has gradually decreased from 51.7 % in 1973 to 16.3 % in 1998 , in absolute figures from 382 cases in 1973 decreased to 60 cases in 1998 .
	manualset3
161032	5	411839	7	NULL	NULL	0	NULL	51.7 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of occupational skin diseases in relation to all occupational diseases has gradually decreased from 51.7 % in 1973 to 16.3 % in 1998 , in absolute figures from 382 cases in 1973 decreased to 60 cases in 1998 .
	manualset3
161033	6	411839	7	NULL	NULL	0	NULL	1973	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of occupational skin diseases in relation to all occupational diseases has gradually decreased from 51.7 % in 1973 to 16.3 % in 1998 , in absolute figures from 382 cases in 1973 decreased to 60 cases in 1998 .
	manualset3
161034	7	411839	7	NULL	NULL	0	NULL	16.3 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of occupational skin diseases in relation to all occupational diseases has gradually decreased from 51.7 % in 1973 to 16.3 % in 1998 , in absolute figures from 382 cases in 1973 decreased to 60 cases in 1998 .
	manualset3
161035	8	411839	7	NULL	NULL	0	NULL	1998	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of occupational skin diseases in relation to all occupational diseases has gradually decreased from 51.7 % in 1973 to 16.3 % in 1998 , in absolute figures from 382 cases in 1973 decreased to 60 cases in 1998 .
	manualset3
161036	9	411839	7	NULL	NULL	0	NULL	absolute figures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of occupational skin diseases in relation to all occupational diseases has gradually decreased from 51.7 % in 1973 to 16.3 % in 1998 , in absolute figures from 382 cases in 1973 decreased to 60 cases in 1998 .
	manualset3
161037	10	411839	7	NULL	NULL	0	NULL	382 cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of occupational skin diseases in relation to all occupational diseases has gradually decreased from 51.7 % in 1973 to 16.3 % in 1998 , in absolute figures from 382 cases in 1973 decreased to 60 cases in 1998 .
	manualset3
161038	11	411839	7	NULL	NULL	0	NULL	1973	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of occupational skin diseases in relation to all occupational diseases has gradually decreased from 51.7 % in 1973 to 16.3 % in 1998 , in absolute figures from 382 cases in 1973 decreased to 60 cases in 1998 .
	manualset3
161039	12	411839	7	NULL	NULL	0	NULL	60 cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of occupational skin diseases in relation to all occupational diseases has gradually decreased from 51.7 % in 1973 to 16.3 % in 1998 , in absolute figures from 382 cases in 1973 decreased to 60 cases in 1998 .
	manualset3
161040	13	411839	7	NULL	NULL	0	NULL	1998	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of occupational skin diseases in relation to all occupational diseases has gradually decreased from 51.7 % in 1973 to 16.3 % in 1998 , in absolute figures from 382 cases in 1973 decreased to 60 cases in 1998 .
	manualset3
161041	1	411840	7	NULL	NULL	0	NULL	proportion	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of vascularized zone to avascular zone depends on the age of the subject and , in newborns , is approximately 33 % .
	manualset3
161042	2	411840	7	NULL	NULL	0	NULL	vascularized zone	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of vascularized zone to avascular zone depends on the age of the subject and , in newborns , is approximately 33 % .
	manualset3
161043	3	411840	7	NULL	NULL	0	NULL	 avascular zone	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of vascularized zone to avascular zone depends on the age of the subject and , in newborns , is approximately 33 % .
	manualset3
161044	4	411840	7	NULL	NULL	NULL	NULL	age	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proportion of vascularized zone to avascular zone depends on the age of the subject and , in newborns , is approximately 33 % .
	manualset3
161045	5	411840	7	NULL	NULL	0	NULL	subject 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of vascularized zone to avascular zone depends on the age of the subject and , in newborns , is approximately 33 % .
	manualset3
161046	6	411840	7	NULL	NULL	0	NULL	newborns	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of vascularized zone to avascular zone depends on the age of the subject and , in newborns , is approximately 33 % .
	manualset3
161047	7	411840	7	NULL	NULL	0	NULL	33 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportion of vascularized zone to avascular zone depends on the age of the subject and , in newborns , is approximately 33 % .
	manualset3
161048	1	411841	7	NULL	NULL	NULL	NULL	 approach 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proposed approach for quantifying sources of error provides a crucial step that is required in the development of experimentally based dynamic models designed to examine and test hypotheses regarding multijoint control logic .
	manualset3
161049	2	411841	7	NULL	NULL	NULL	NULL	sources of error	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proposed approach for quantifying sources of error provides a crucial step that is required in the development of experimentally based dynamic models designed to examine and test hypotheses regarding multijoint control logic .
	manualset3
161050	3	411841	7	NULL	NULL	0	NULL	 development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed approach for quantifying sources of error provides a crucial step that is required in the development of experimentally based dynamic models designed to examine and test hypotheses regarding multijoint control logic .
	manualset3
161051	4	411841	7	NULL	NULL	NULL	NULL	experimentally based dynamic models	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proposed approach for quantifying sources of error provides a crucial step that is required in the development of experimentally based dynamic models designed to examine and test hypotheses regarding multijoint control logic .
	manualset3
161052	5	411841	7	NULL	NULL	NULL	NULL	 hypotheses	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proposed approach for quantifying sources of error provides a crucial step that is required in the development of experimentally based dynamic models designed to examine and test hypotheses regarding multijoint control logic .
	manualset3
161053	6	411841	7	NULL	NULL	0	NULL	multijoint control logic	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed approach for quantifying sources of error provides a crucial step that is required in the development of experimentally based dynamic models designed to examine and test hypotheses regarding multijoint control logic .
	manualset3
162355	7	411841	7	NULL	NULL	0	NULL	crucial step	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed approach for quantifying sources of error provides a crucial step that is required in the development of experimentally based dynamic models designed to examine and test hypotheses regarding multijoint control logic .
	manualset3
161054	1	411842	7	NULL	NULL	0	NULL	kinetic model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed kinetic model takes into account ( i ) triggering of the effector function in cells in the vicinity of transformed cells , ( ii ) intercellular signalling between effector and transformed cells and ( iii ) execution of apoptosis in attacked cells .
	manualset3
161055	2	411842	7	NULL	NULL	0	NULL	effector function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed kinetic model takes into account ( i ) triggering of the effector function in cells in the vicinity of transformed cells , ( ii ) intercellular signalling between effector and transformed cells and ( iii ) execution of apoptosis in attacked cells .
	manualset3
161056	3	411842	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed kinetic model takes into account ( i ) triggering of the effector function in cells in the vicinity of transformed cells , ( ii ) intercellular signalling between effector and transformed cells and ( iii ) execution of apoptosis in attacked cells .
	manualset3
161057	4	411842	7	NULL	NULL	0	NULL	transformed cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed kinetic model takes into account ( i ) triggering of the effector function in cells in the vicinity of transformed cells , ( ii ) intercellular signalling between effector and transformed cells and ( iii ) execution of apoptosis in attacked cells .
	manualset3
161058	5	411842	7	NULL	NULL	0	NULL	intercellular signalling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed kinetic model takes into account ( i ) triggering of the effector function in cells in the vicinity of transformed cells , ( ii ) intercellular signalling between effector and transformed cells and ( iii ) execution of apoptosis in attacked cells .
	manualset3
161059	6	411842	7	NULL	NULL	NULL	NULL	effector	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proposed kinetic model takes into account ( i ) triggering of the effector function in cells in the vicinity of transformed cells , ( ii ) intercellular signalling between effector and transformed cells and ( iii ) execution of apoptosis in attacked cells .
	manualset3
161060	7	411842	7	NULL	NULL	0	NULL	transformed cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed kinetic model takes into account ( i ) triggering of the effector function in cells in the vicinity of transformed cells , ( ii ) intercellular signalling between effector and transformed cells and ( iii ) execution of apoptosis in attacked cells .
	manualset3
161061	8	411842	7	NULL	NULL	0	NULL	execution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed kinetic model takes into account ( i ) triggering of the effector function in cells in the vicinity of transformed cells , ( ii ) intercellular signalling between effector and transformed cells and ( iii ) execution of apoptosis in attacked cells .
	manualset3
161062	9	411842	7	NULL	NULL	0	NULL	apoptosis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed kinetic model takes into account ( i ) triggering of the effector function in cells in the vicinity of transformed cells , ( ii ) intercellular signalling between effector and transformed cells and ( iii ) execution of apoptosis in attacked cells .
	manualset3
161063	10	411842	7	NULL	NULL	0	NULL	attacked cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed kinetic model takes into account ( i ) triggering of the effector function in cells in the vicinity of transformed cells , ( ii ) intercellular signalling between effector and transformed cells and ( iii ) execution of apoptosis in attacked cells .
	manualset3
169445	11	411842	7	NULL	NULL	0	NULL	vicinity	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed kinetic model takes into account ( i ) triggering of the effector function in cells in the vicinity of transformed cells , ( ii ) intercellular signalling between effector and transformed cells and ( iii ) execution of apoptosis in attacked cells .
	manualset3
161064	1	411843	7	NULL	NULL	0	NULL	AVR4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	AVR4 increased the levels of PA and DGPP in a Cf-4 ( + ) - , time - and dose-dependent manner , while the non-matching elicitor AVR9 did not trigger any response .
	manualset3
161065	2	411843	7	NULL	NULL	0	NULL	levels of PA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	AVR4 increased the levels of PA and DGPP in a Cf-4 ( + ) - , time - and dose-dependent manner , while the non-matching elicitor AVR9 did not trigger any response .
	manualset3
161066	3	411843	7	NULL	NULL	0	NULL	levels of DGPP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	AVR4 increased the levels of PA and DGPP in a Cf-4 ( + ) - , time - and dose-dependent manner , while the non-matching elicitor AVR9 did not trigger any response .
	manualset3
161067	4	411843	7	NULL	NULL	0	NULL	Cf-4 ( + ) -	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	AVR4 increased the levels of PA and DGPP in a Cf-4 ( + ) - , time - and dose-dependent manner , while the non-matching elicitor AVR9 did not trigger any response .
	manualset3
161068	5	411843	7	NULL	NULL	0	NULL	time -	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	AVR4 increased the levels of PA and DGPP in a Cf-4 ( + ) - , time - and dose-dependent manner , while the non-matching elicitor AVR9 did not trigger any response .
	manualset3
161069	6	411843	7	NULL	NULL	0	NULL	dose-dependent manner	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	AVR4 increased the levels of PA and DGPP in a Cf-4 ( + ) - , time - and dose-dependent manner , while the non-matching elicitor AVR9 did not trigger any response .
	manualset3
161070	7	411843	7	NULL	NULL	0	NULL	elicitor AVR9	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	AVR4 increased the levels of PA and DGPP in a Cf-4 ( + ) - , time - and dose-dependent manner , while the non-matching elicitor AVR9 did not trigger any response .
	manualset3
161071	8	411843	7	NULL	NULL	0	NULL	response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	AVR4 increased the levels of PA and DGPP in a Cf-4 ( + ) - , time - and dose-dependent manner , while the non-matching elicitor AVR9 did not trigger any response .
	manualset3
161072	1	411844	7	NULL	NULL	0	NULL	method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed method proved to have satisfactory recovery , precision and accuracy .
	manualset3
161073	2	411844	7	NULL	NULL	NULL	NULL	recovery	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proposed method proved to have satisfactory recovery , precision and accuracy .
	manualset3
161074	3	411844	7	NULL	NULL	NULL	NULL	precision	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proposed method proved to have satisfactory recovery , precision and accuracy .
	manualset3
161075	4	411844	7	NULL	NULL	NULL	NULL	accuracy	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proposed method proved to have satisfactory recovery , precision and accuracy .
	manualset3
161076	1	411845	7	NULL	NULL	0	NULL	 pathophysiology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed pathophysiology of PPTTN is largely based on studies in spinal nerve injury models .
	manualset3
161077	2	411845	7	NULL	NULL	0	NULL	PPTTN	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed pathophysiology of PPTTN is largely based on studies in spinal nerve injury models .
	manualset3
161078	3	411845	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed pathophysiology of PPTTN is largely based on studies in spinal nerve injury models .
	manualset3
161079	4	411845	7	NULL	NULL	0	NULL	spinal nerve injury models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed pathophysiology of PPTTN is largely based on studies in spinal nerve injury models .
	manualset3
161080	1	411846	7	NULL	NULL	0	NULL	definition	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed working definition of disease modification resulting from the group discussions was `` an improvement in , or stabilization of , structural or functional parameters as a result of reduction in the rate of progression of these parameters which occurs whilst an intervention is applied and may persist even if the intervention is withdrawn '' .
	manualset3
161081	2	411846	7	NULL	NULL	0	NULL	disease modification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed working definition of disease modification resulting from the group discussions was `` an improvement in , or stabilization of , structural or functional parameters as a result of reduction in the rate of progression of these parameters which occurs whilst an intervention is applied and may persist even if the intervention is withdrawn '' .
	manualset3
161082	3	411846	7	NULL	NULL	0	NULL	 group discussions	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed working definition of disease modification resulting from the group discussions was `` an improvement in , or stabilization of , structural or functional parameters as a result of reduction in the rate of progression of these parameters which occurs whilst an intervention is applied and may persist even if the intervention is withdrawn '' .
	manualset3
161083	4	411846	7	NULL	NULL	NULL	NULL	improvement	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proposed working definition of disease modification resulting from the group discussions was `` an improvement in , or stabilization of , structural or functional parameters as a result of reduction in the rate of progression of these parameters which occurs whilst an intervention is applied and may persist even if the intervention is withdrawn '' .
	manualset3
161084	5	411846	7	NULL	NULL	0	NULL	stabilization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed working definition of disease modification resulting from the group discussions was `` an improvement in , or stabilization of , structural or functional parameters as a result of reduction in the rate of progression of these parameters which occurs whilst an intervention is applied and may persist even if the intervention is withdrawn '' .
	manualset3
161085	6	411846	7	NULL	NULL	NULL	NULL	structural parameters	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proposed working definition of disease modification resulting from the group discussions was `` an improvement in , or stabilization of , structural or functional parameters as a result of reduction in the rate of progression of these parameters which occurs whilst an intervention is applied and may persist even if the intervention is withdrawn '' .
	manualset3
161086	7	411846	7	NULL	NULL	NULL	NULL	 functional parameters	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proposed working definition of disease modification resulting from the group discussions was `` an improvement in , or stabilization of , structural or functional parameters as a result of reduction in the rate of progression of these parameters which occurs whilst an intervention is applied and may persist even if the intervention is withdrawn '' .
	manualset3
161087	8	411846	7	NULL	NULL	0	NULL	result	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed working definition of disease modification resulting from the group discussions was `` an improvement in , or stabilization of , structural or functional parameters as a result of reduction in the rate of progression of these parameters which occurs whilst an intervention is applied and may persist even if the intervention is withdrawn '' .
	manualset3
161088	9	411846	7	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed working definition of disease modification resulting from the group discussions was `` an improvement in , or stabilization of , structural or functional parameters as a result of reduction in the rate of progression of these parameters which occurs whilst an intervention is applied and may persist even if the intervention is withdrawn '' .
	manualset3
161089	10	411846	7	NULL	NULL	0	NULL	rate of progression	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed working definition of disease modification resulting from the group discussions was `` an improvement in , or stabilization of , structural or functional parameters as a result of reduction in the rate of progression of these parameters which occurs whilst an intervention is applied and may persist even if the intervention is withdrawn '' .
	manualset3
161090	11	411846	7	NULL	NULL	NULL	NULL	parameters 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proposed working definition of disease modification resulting from the group discussions was `` an improvement in , or stabilization of , structural or functional parameters as a result of reduction in the rate of progression of these parameters which occurs whilst an intervention is applied and may persist even if the intervention is withdrawn '' .
	manualset3
161091	12	411846	7	NULL	NULL	0	NULL	intervention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed working definition of disease modification resulting from the group discussions was `` an improvement in , or stabilization of , structural or functional parameters as a result of reduction in the rate of progression of these parameters which occurs whilst an intervention is applied and may persist even if the intervention is withdrawn '' .
	manualset3
161092	13	411846	7	NULL	NULL	0	NULL	intervention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed working definition of disease modification resulting from the group discussions was `` an improvement in , or stabilization of , structural or functional parameters as a result of reduction in the rate of progression of these parameters which occurs whilst an intervention is applied and may persist even if the intervention is withdrawn '' .
	manualset3
161093	1	411847	7	NULL	NULL	0	NULL	proprotein convertases ( PCs )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The proprotein convertases ( PCs ) participate in the limited proteolysis of integrin alpha4 subunit at the H ( 592 ) VISKR ( 597 ) downward arrow ST site ( where underlined residues indicate positively charged amino acids important for PC-mediated cleavage and downward arrow indicates the cleavage site ) , since this cleavage is inhibited by the serpin alpha1-PDX ( alpha1-antitrypsin Portland ) .
	manualset3
161094	2	411847	7	NULL	NULL	0	NULL	limited proteolysis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The proprotein convertases ( PCs ) participate in the limited proteolysis of integrin alpha4 subunit at the H ( 592 ) VISKR ( 597 ) downward arrow ST site ( where underlined residues indicate positively charged amino acids important for PC-mediated cleavage and downward arrow indicates the cleavage site ) , since this cleavage is inhibited by the serpin alpha1-PDX ( alpha1-antitrypsin Portland ) .
	manualset3
161095	3	411847	7	NULL	NULL	0	NULL	integrin alpha4 subunit	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proprotein convertases ( PCs ) participate in the limited proteolysis of integrin alpha4 subunit at the H ( 592 ) VISKR ( 597 ) downward arrow ST site ( where underlined residues indicate positively charged amino acids important for PC-mediated cleavage and downward arrow indicates the cleavage site ) , since this cleavage is inhibited by the serpin alpha1-PDX ( alpha1-antitrypsin Portland ) .
	manualset3
161096	4	411847	7	NULL	NULL	0	NULL	H ( 592 ) VISKR ( 597 )	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The proprotein convertases ( PCs ) participate in the limited proteolysis of integrin alpha4 subunit at the H ( 592 ) VISKR ( 597 ) downward arrow ST site ( where underlined residues indicate positively charged amino acids important for PC-mediated cleavage and downward arrow indicates the cleavage site ) , since this cleavage is inhibited by the serpin alpha1-PDX ( alpha1-antitrypsin Portland ) .
	manualset3
161097	5	411847	7	NULL	NULL	NULL	NULL	ST site 	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proprotein convertases ( PCs ) participate in the limited proteolysis of integrin alpha4 subunit at the H ( 592 ) VISKR ( 597 ) downward arrow ST site ( where underlined residues indicate positively charged amino acids important for PC-mediated cleavage and downward arrow indicates the cleavage site ) , since this cleavage is inhibited by the serpin alpha1-PDX ( alpha1-antitrypsin Portland ) .
	manualset3
161098	6	411847	7	NULL	NULL	0	NULL	underlined residues 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The proprotein convertases ( PCs ) participate in the limited proteolysis of integrin alpha4 subunit at the H ( 592 ) VISKR ( 597 ) downward arrow ST site ( where underlined residues indicate positively charged amino acids important for PC-mediated cleavage and downward arrow indicates the cleavage site ) , since this cleavage is inhibited by the serpin alpha1-PDX ( alpha1-antitrypsin Portland ) .
	manualset3
161099	7	411847	7	NULL	NULL	0	NULL	positively charged amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The proprotein convertases ( PCs ) participate in the limited proteolysis of integrin alpha4 subunit at the H ( 592 ) VISKR ( 597 ) downward arrow ST site ( where underlined residues indicate positively charged amino acids important for PC-mediated cleavage and downward arrow indicates the cleavage site ) , since this cleavage is inhibited by the serpin alpha1-PDX ( alpha1-antitrypsin Portland ) .
	manualset3
161100	8	411847	7	NULL	NULL	0	NULL	PC-mediated cleavage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The proprotein convertases ( PCs ) participate in the limited proteolysis of integrin alpha4 subunit at the H ( 592 ) VISKR ( 597 ) downward arrow ST site ( where underlined residues indicate positively charged amino acids important for PC-mediated cleavage and downward arrow indicates the cleavage site ) , since this cleavage is inhibited by the serpin alpha1-PDX ( alpha1-antitrypsin Portland ) .
	manualset3
161101	9	411847	7	NULL	NULL	NULL	NULL	downward arrow 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proprotein convertases ( PCs ) participate in the limited proteolysis of integrin alpha4 subunit at the H ( 592 ) VISKR ( 597 ) downward arrow ST site ( where underlined residues indicate positively charged amino acids important for PC-mediated cleavage and downward arrow indicates the cleavage site ) , since this cleavage is inhibited by the serpin alpha1-PDX ( alpha1-antitrypsin Portland ) .
	manualset3
161102	10	411847	7	NULL	NULL	0	NULL	cleavage site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proprotein convertases ( PCs ) participate in the limited proteolysis of integrin alpha4 subunit at the H ( 592 ) VISKR ( 597 ) downward arrow ST site ( where underlined residues indicate positively charged amino acids important for PC-mediated cleavage and downward arrow indicates the cleavage site ) , since this cleavage is inhibited by the serpin alpha1-PDX ( alpha1-antitrypsin Portland ) .
	manualset3
161103	11	411847	7	NULL	NULL	0	NULL	cleavage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The proprotein convertases ( PCs ) participate in the limited proteolysis of integrin alpha4 subunit at the H ( 592 ) VISKR ( 597 ) downward arrow ST site ( where underlined residues indicate positively charged amino acids important for PC-mediated cleavage and downward arrow indicates the cleavage site ) , since this cleavage is inhibited by the serpin alpha1-PDX ( alpha1-antitrypsin Portland ) .
	manualset3
161104	12	411847	7	NULL	NULL	0	NULL	serpin alpha1-PDX	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proprotein convertases ( PCs ) participate in the limited proteolysis of integrin alpha4 subunit at the H ( 592 ) VISKR ( 597 ) downward arrow ST site ( where underlined residues indicate positively charged amino acids important for PC-mediated cleavage and downward arrow indicates the cleavage site ) , since this cleavage is inhibited by the serpin alpha1-PDX ( alpha1-antitrypsin Portland ) .
	manualset3
161105	13	411847	7	NULL	NULL	0	NULL	alpha1-antitrypsin Portland	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proprotein convertases ( PCs ) participate in the limited proteolysis of integrin alpha4 subunit at the H ( 592 ) VISKR ( 597 ) downward arrow ST site ( where underlined residues indicate positively charged amino acids important for PC-mediated cleavage and downward arrow indicates the cleavage site ) , since this cleavage is inhibited by the serpin alpha1-PDX ( alpha1-antitrypsin Portland ) .
	manualset3
161106	14	411847	7	NULL	NULL	0	NULL	downward arrow	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proprotein convertases ( PCs ) participate in the limited proteolysis of integrin alpha4 subunit at the H ( 592 ) VISKR ( 597 ) downward arrow ST site ( where underlined residues indicate positively charged amino acids important for PC-mediated cleavage and downward arrow indicates the cleavage site ) , since this cleavage is inhibited by the serpin alpha1-PDX ( alpha1-antitrypsin Portland ) .
	manualset3
161107	1	411848	7	NULL	NULL	0	NULL	proteases	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteases are predominantly acid proteases and have optimal temperature for activity at around 45 degrees C. Their activity could be partially inhibited by protease inhibitors , indicating the existence of at least four kinds of proteases in these culture fluids , aspartic - , serine - , cysteine - , and metallo-proteases .
	manualset3
161108	2	411848	7	NULL	NULL	0	NULL	acid proteases	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteases are predominantly acid proteases and have optimal temperature for activity at around 45 degrees C. Their activity could be partially inhibited by protease inhibitors , indicating the existence of at least four kinds of proteases in these culture fluids , aspartic - , serine - , cysteine - , and metallo-proteases .
	manualset3
161109	3	411848	7	NULL	NULL	0	NULL	optimal temperature	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteases are predominantly acid proteases and have optimal temperature for activity at around 45 degrees C. Their activity could be partially inhibited by protease inhibitors , indicating the existence of at least four kinds of proteases in these culture fluids , aspartic - , serine - , cysteine - , and metallo-proteases .
	manualset3
161110	4	411848	7	NULL	NULL	NULL	NULL	activity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proteases are predominantly acid proteases and have optimal temperature for activity at around 45 degrees C. Their activity could be partially inhibited by protease inhibitors , indicating the existence of at least four kinds of proteases in these culture fluids , aspartic - , serine - , cysteine - , and metallo-proteases .
	manualset3
161111	5	411848	7	NULL	NULL	0	NULL	45 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteases are predominantly acid proteases and have optimal temperature for activity at around 45 degrees C. Their activity could be partially inhibited by protease inhibitors , indicating the existence of at least four kinds of proteases in these culture fluids , aspartic - , serine - , cysteine - , and metallo-proteases .
	manualset3
161112	6	411848	7	NULL	NULL	0	NULL	activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteases are predominantly acid proteases and have optimal temperature for activity at around 45 degrees C. Their activity could be partially inhibited by protease inhibitors , indicating the existence of at least four kinds of proteases in these culture fluids , aspartic - , serine - , cysteine - , and metallo-proteases .
	manualset3
161113	7	411848	7	NULL	NULL	0	NULL	protease inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteases are predominantly acid proteases and have optimal temperature for activity at around 45 degrees C. Their activity could be partially inhibited by protease inhibitors , indicating the existence of at least four kinds of proteases in these culture fluids , aspartic - , serine - , cysteine - , and metallo-proteases .
	manualset3
161114	8	411848	7	NULL	NULL	0	NULL	existence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteases are predominantly acid proteases and have optimal temperature for activity at around 45 degrees C. Their activity could be partially inhibited by protease inhibitors , indicating the existence of at least four kinds of proteases in these culture fluids , aspartic - , serine - , cysteine - , and metallo-proteases .
	manualset3
161115	9	411848	7	NULL	NULL	0	NULL	proteases	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteases are predominantly acid proteases and have optimal temperature for activity at around 45 degrees C. Their activity could be partially inhibited by protease inhibitors , indicating the existence of at least four kinds of proteases in these culture fluids , aspartic - , serine - , cysteine - , and metallo-proteases .
	manualset3
161116	10	411848	7	NULL	NULL	NULL	NULL	culture fluids	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proteases are predominantly acid proteases and have optimal temperature for activity at around 45 degrees C. Their activity could be partially inhibited by protease inhibitors , indicating the existence of at least four kinds of proteases in these culture fluids , aspartic - , serine - , cysteine - , and metallo-proteases .
	manualset3
161117	11	411848	7	NULL	NULL	0	NULL	aspartic protease	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteases are predominantly acid proteases and have optimal temperature for activity at around 45 degrees C. Their activity could be partially inhibited by protease inhibitors , indicating the existence of at least four kinds of proteases in these culture fluids , aspartic - , serine - , cysteine - , and metallo-proteases .
	manualset3
161118	12	411848	7	NULL	NULL	0	NULL	 serine protease	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteases are predominantly acid proteases and have optimal temperature for activity at around 45 degrees C. Their activity could be partially inhibited by protease inhibitors , indicating the existence of at least four kinds of proteases in these culture fluids , aspartic - , serine - , cysteine - , and metallo-proteases .
	manualset3
161119	13	411848	7	NULL	NULL	0	NULL	cysteine protease	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteases are predominantly acid proteases and have optimal temperature for activity at around 45 degrees C. Their activity could be partially inhibited by protease inhibitors , indicating the existence of at least four kinds of proteases in these culture fluids , aspartic - , serine - , cysteine - , and metallo-proteases .
	manualset3
161120	14	411848	7	NULL	NULL	0	NULL	metallo-proteases	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteases are predominantly acid proteases and have optimal temperature for activity at around 45 degrees C. Their activity could be partially inhibited by protease inhibitors , indicating the existence of at least four kinds of proteases in these culture fluids , aspartic - , serine - , cysteine - , and metallo-proteases .
	manualset3
161121	1	411849	7	NULL	NULL	0	NULL	 protective efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The protective efficacy of the HSV-1 ISCOM vaccine is compared with that of a purified , aqueous HSV-1 antigen preparation administered using a similar immunization schedule .
	manualset3
161122	2	411849	7	NULL	NULL	0	NULL	HSV-1 ISCOM vaccine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The protective efficacy of the HSV-1 ISCOM vaccine is compared with that of a purified , aqueous HSV-1 antigen preparation administered using a similar immunization schedule .
	manualset3
161123	3	411849	7	NULL	NULL	0	NULL	aqueous HSV-1 antigen preparation	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The protective efficacy of the HSV-1 ISCOM vaccine is compared with that of a purified , aqueous HSV-1 antigen preparation administered using a similar immunization schedule .
	manualset3
161124	4	411849	7	NULL	NULL	0	NULL	immunization schedule	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The protective efficacy of the HSV-1 ISCOM vaccine is compared with that of a purified , aqueous HSV-1 antigen preparation administered using a similar immunization schedule .
	manualset3
161125	1	411850	7	NULL	NULL	0	NULL	protein ( TbFPPS )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein ( TbFPPS ) is an attractive target for drug development because the growth of T. brucei has been shown to be inhibited by analogs of its substrates , the nitrogen containing bisphosphonates currently in use in bone resorption therapy .
	manualset3
161126	2	411850	7	NULL	NULL	0	NULL	target	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein ( TbFPPS ) is an attractive target for drug development because the growth of T. brucei has been shown to be inhibited by analogs of its substrates , the nitrogen containing bisphosphonates currently in use in bone resorption therapy .
	manualset3
161127	3	411850	7	NULL	NULL	0	NULL	drug development	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein ( TbFPPS ) is an attractive target for drug development because the growth of T. brucei has been shown to be inhibited by analogs of its substrates , the nitrogen containing bisphosphonates currently in use in bone resorption therapy .
	manualset3
161128	4	411850	7	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein ( TbFPPS ) is an attractive target for drug development because the growth of T. brucei has been shown to be inhibited by analogs of its substrates , the nitrogen containing bisphosphonates currently in use in bone resorption therapy .
	manualset3
161129	5	411850	7	NULL	NULL	0	NULL	T. brucei	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein ( TbFPPS ) is an attractive target for drug development because the growth of T. brucei has been shown to be inhibited by analogs of its substrates , the nitrogen containing bisphosphonates currently in use in bone resorption therapy .
	manualset3
161130	6	411850	7	NULL	NULL	0	NULL	analogs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein ( TbFPPS ) is an attractive target for drug development because the growth of T. brucei has been shown to be inhibited by analogs of its substrates , the nitrogen containing bisphosphonates currently in use in bone resorption therapy .
	manualset3
161131	7	411850	7	NULL	NULL	0	NULL	substrates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein ( TbFPPS ) is an attractive target for drug development because the growth of T. brucei has been shown to be inhibited by analogs of its substrates , the nitrogen containing bisphosphonates currently in use in bone resorption therapy .
	manualset3
161132	8	411850	7	NULL	NULL	0	NULL	nitrogen containing bisphosphonates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein ( TbFPPS ) is an attractive target for drug development because the growth of T. brucei has been shown to be inhibited by analogs of its substrates , the nitrogen containing bisphosphonates currently in use in bone resorption therapy .
	manualset3
161133	9	411850	7	NULL	NULL	0	NULL	bone resorption therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein ( TbFPPS ) is an attractive target for drug development because the growth of T. brucei has been shown to be inhibited by analogs of its substrates , the nitrogen containing bisphosphonates currently in use in bone resorption therapy .
	manualset3
161134	1	411851	7	NULL	NULL	0	NULL	protein concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein concentrations in the crude cytosolic extracts prior to elution of PKC through DE-52 columns were significantly increased in the AM/PC ( by 11 % , P less than 0.05 ) and right HIPP ( by 18 % , P less than 0.02 ) 4 weeks after the last seizure .
	manualset3
161135	2	411851	7	NULL	NULL	0	NULL	crude cytosolic extracts	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein concentrations in the crude cytosolic extracts prior to elution of PKC through DE-52 columns were significantly increased in the AM/PC ( by 11 % , P less than 0.05 ) and right HIPP ( by 18 % , P less than 0.02 ) 4 weeks after the last seizure .
	manualset3
161136	3	411851	7	NULL	NULL	0	NULL	PKC	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein concentrations in the crude cytosolic extracts prior to elution of PKC through DE-52 columns were significantly increased in the AM/PC ( by 11 % , P less than 0.05 ) and right HIPP ( by 18 % , P less than 0.02 ) 4 weeks after the last seizure .
	manualset3
161137	4	411851	7	NULL	NULL	0	NULL	DE-52 columns	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein concentrations in the crude cytosolic extracts prior to elution of PKC through DE-52 columns were significantly increased in the AM/PC ( by 11 % , P less than 0.05 ) and right HIPP ( by 18 % , P less than 0.02 ) 4 weeks after the last seizure .
	manualset3
161138	5	411851	7	NULL	NULL	0	NULL	 AM/PC	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein concentrations in the crude cytosolic extracts prior to elution of PKC through DE-52 columns were significantly increased in the AM/PC ( by 11 % , P less than 0.05 ) and right HIPP ( by 18 % , P less than 0.02 ) 4 weeks after the last seizure .
	manualset3
161139	6	411851	7	NULL	NULL	0	NULL	11 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein concentrations in the crude cytosolic extracts prior to elution of PKC through DE-52 columns were significantly increased in the AM/PC ( by 11 % , P less than 0.05 ) and right HIPP ( by 18 % , P less than 0.02 ) 4 weeks after the last seizure .
	manualset3
161140	7	411851	7	NULL	NULL	0	NULL	P less than 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein concentrations in the crude cytosolic extracts prior to elution of PKC through DE-52 columns were significantly increased in the AM/PC ( by 11 % , P less than 0.05 ) and right HIPP ( by 18 % , P less than 0.02 ) 4 weeks after the last seizure .
	manualset3
161141	8	411851	7	NULL	NULL	0	NULL	 right HIPP	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein concentrations in the crude cytosolic extracts prior to elution of PKC through DE-52 columns were significantly increased in the AM/PC ( by 11 % , P less than 0.05 ) and right HIPP ( by 18 % , P less than 0.02 ) 4 weeks after the last seizure .
	manualset3
161142	9	411851	7	NULL	NULL	0	NULL	18 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein concentrations in the crude cytosolic extracts prior to elution of PKC through DE-52 columns were significantly increased in the AM/PC ( by 11 % , P less than 0.05 ) and right HIPP ( by 18 % , P less than 0.02 ) 4 weeks after the last seizure .
	manualset3
161143	10	411851	7	NULL	NULL	0	NULL	P less than 0.02	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein concentrations in the crude cytosolic extracts prior to elution of PKC through DE-52 columns were significantly increased in the AM/PC ( by 11 % , P less than 0.05 ) and right HIPP ( by 18 % , P less than 0.02 ) 4 weeks after the last seizure .
	manualset3
161144	11	411851	7	NULL	NULL	0	NULL	 4 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein concentrations in the crude cytosolic extracts prior to elution of PKC through DE-52 columns were significantly increased in the AM/PC ( by 11 % , P less than 0.05 ) and right HIPP ( by 18 % , P less than 0.02 ) 4 weeks after the last seizure .
	manualset3
161146	12	411851	7	NULL	NULL	0	NULL	seizure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein concentrations in the crude cytosolic extracts prior to elution of PKC through DE-52 columns were significantly increased in the AM/PC ( by 11 % , P less than 0.05 ) and right HIPP ( by 18 % , P less than 0.02 ) 4 weeks after the last seizure .
	manualset3
161147	1	411852	7	NULL	NULL	0	NULL	AW1	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	AW1 did not produce siderophore activity when cultured in tomato xylem sap , suggesting that the main location in tomato for R. solanacearum during pathogenesis is iron replete .
	manualset3
161148	2	411852	7	NULL	NULL	0	NULL	siderophore activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	AW1 did not produce siderophore activity when cultured in tomato xylem sap , suggesting that the main location in tomato for R. solanacearum during pathogenesis is iron replete .
	manualset3
161149	3	411852	7	NULL	NULL	0	NULL	 tomato xylem sap 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	AW1 did not produce siderophore activity when cultured in tomato xylem sap , suggesting that the main location in tomato for R. solanacearum during pathogenesis is iron replete .
	manualset3
161150	4	411852	7	NULL	NULL	0	NULL	 location	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	AW1 did not produce siderophore activity when cultured in tomato xylem sap , suggesting that the main location in tomato for R. solanacearum during pathogenesis is iron replete .
	manualset3
161151	5	411852	7	NULL	NULL	0	NULL	tomato	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	AW1 did not produce siderophore activity when cultured in tomato xylem sap , suggesting that the main location in tomato for R. solanacearum during pathogenesis is iron replete .
	manualset3
161152	6	411852	7	NULL	NULL	0	NULL	R. solanacearum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	AW1 did not produce siderophore activity when cultured in tomato xylem sap , suggesting that the main location in tomato for R. solanacearum during pathogenesis is iron replete .
	manualset3
161153	7	411852	7	NULL	NULL	0	NULL	pathogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	AW1 did not produce siderophore activity when cultured in tomato xylem sap , suggesting that the main location in tomato for R. solanacearum during pathogenesis is iron replete .
	manualset3
162356	8	411852	7	NULL	NULL	0	NULL	iron	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	AW1 did not produce siderophore activity when cultured in tomato xylem sap , suggesting that the main location in tomato for R. solanacearum during pathogenesis is iron replete .
	manualset3
161154	1	411853	7	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein is present on most or all of the RF DNA , including actively replicating molecules , and is associated with the 5 ' - terminal endonuclease Hae III fragments of both the viral and complementary strands of RF .
	manualset3
161155	2	411853	7	NULL	NULL	0	NULL	RF DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein is present on most or all of the RF DNA , including actively replicating molecules , and is associated with the 5 ' - terminal endonuclease Hae III fragments of both the viral and complementary strands of RF .
	manualset3
161156	3	411853	7	NULL	NULL	NULL	NULL	replicating molecules	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The protein is present on most or all of the RF DNA , including actively replicating molecules , and is associated with the 5 ' - terminal endonuclease Hae III fragments of both the viral and complementary strands of RF .
	manualset3
161157	4	411853	7	NULL	NULL	0	NULL	5 ' - terminal endonuclease Hae III fragments	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein is present on most or all of the RF DNA , including actively replicating molecules , and is associated with the 5 ' - terminal endonuclease Hae III fragments of both the viral and complementary strands of RF .
	manualset3
161158	5	411853	7	NULL	NULL	0	NULL	viral strands	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein is present on most or all of the RF DNA , including actively replicating molecules , and is associated with the 5 ' - terminal endonuclease Hae III fragments of both the viral and complementary strands of RF .
	manualset3
161159	6	411853	7	NULL	NULL	0	NULL	complementary strands	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein is present on most or all of the RF DNA , including actively replicating molecules , and is associated with the 5 ' - terminal endonuclease Hae III fragments of both the viral and complementary strands of RF .
	manualset3
161160	7	411853	7	NULL	NULL	0	NULL	RF	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein is present on most or all of the RF DNA , including actively replicating molecules , and is associated with the 5 ' - terminal endonuclease Hae III fragments of both the viral and complementary strands of RF .
	manualset3
161161	1	411854	7	NULL	NULL	0	NULL	protein kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein kinase bound with high affinity to pyruvate kinase type M2 ( Km value for pyruvate kinase = 6 X 10 ( -10 ) M ; it phosphorylated phosvitin and casein but not histones , ATP and GTP were substrates .
	manualset3
161162	2	411854	7	NULL	NULL	0	NULL	pyruvate kinase type M2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein kinase bound with high affinity to pyruvate kinase type M2 ( Km value for pyruvate kinase = 6 X 10 ( -10 ) M ; it phosphorylated phosvitin and casein but not histones , ATP and GTP were substrates .
	manualset3
161163	3	411854	7	NULL	NULL	0	NULL	Km value for pyruvate kinase = 6 X 10 ( -10 ) M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein kinase bound with high affinity to pyruvate kinase type M2 ( Km value for pyruvate kinase = 6 X 10 ( -10 ) M ; it phosphorylated phosvitin and casein but not histones , ATP and GTP were substrates .
	manualset3
161164	4	411854	7	NULL	NULL	0	NULL	phosvitin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein kinase bound with high affinity to pyruvate kinase type M2 ( Km value for pyruvate kinase = 6 X 10 ( -10 ) M ; it phosphorylated phosvitin and casein but not histones , ATP and GTP were substrates .
	manualset3
161165	5	411854	7	NULL	NULL	0	NULL	casein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein kinase bound with high affinity to pyruvate kinase type M2 ( Km value for pyruvate kinase = 6 X 10 ( -10 ) M ; it phosphorylated phosvitin and casein but not histones , ATP and GTP were substrates .
	manualset3
161166	6	411854	7	NULL	NULL	0	NULL	histones	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein kinase bound with high affinity to pyruvate kinase type M2 ( Km value for pyruvate kinase = 6 X 10 ( -10 ) M ; it phosphorylated phosvitin and casein but not histones , ATP and GTP were substrates .
	manualset3
161167	7	411854	7	NULL	NULL	0	NULL	 ATP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein kinase bound with high affinity to pyruvate kinase type M2 ( Km value for pyruvate kinase = 6 X 10 ( -10 ) M ; it phosphorylated phosvitin and casein but not histones , ATP and GTP were substrates .
	manualset3
161168	8	411854	7	NULL	NULL	0	NULL	GTP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein kinase bound with high affinity to pyruvate kinase type M2 ( Km value for pyruvate kinase = 6 X 10 ( -10 ) M ; it phosphorylated phosvitin and casein but not histones , ATP and GTP were substrates .
	manualset3
169454	9	411854	7	NULL	NULL	0	NULL	high affinity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein kinase bound with high affinity to pyruvate kinase type M2 ( Km value for pyruvate kinase = 6 X 10 ( -10 ) M ; it phosphorylated phosvitin and casein but not histones , ATP and GTP were substrates .
	manualset3
161169	1	411855	7	NULL	NULL	0	NULL	protein sequence	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein sequence shows remarkable clusters of charged residues including a long polyglutamic acid tract which presumably constitutes the histone binding site .
	manualset3
161170	2	411855	7	NULL	NULL	0	NULL	charged residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein sequence shows remarkable clusters of charged residues including a long polyglutamic acid tract which presumably constitutes the histone binding site .
	manualset3
161171	3	411855	7	NULL	NULL	0	NULL	long polyglutamic acid tract	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein sequence shows remarkable clusters of charged residues including a long polyglutamic acid tract which presumably constitutes the histone binding site .
	manualset3
161172	4	411855	7	NULL	NULL	0	NULL	histone binding site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein sequence shows remarkable clusters of charged residues including a long polyglutamic acid tract which presumably constitutes the histone binding site .
	manualset3
162357	5	411855	7	NULL	NULL	0	NULL	clusters	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein sequence shows remarkable clusters of charged residues including a long polyglutamic acid tract which presumably constitutes the histone binding site .
	manualset3
161173	1	411856	7	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein showed 27.3-64 .7 % identity to the bacterial sialyltransferases classified into glycosyltransferase family 80 .
	manualset3
161175	2	411856	7	NULL	NULL	0	NULL	27.3-64 .7 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein showed 27.3-64 .7 % identity to the bacterial sialyltransferases classified into glycosyltransferase family 80 .
	manualset3
161176	3	411856	7	NULL	NULL	0	NULL	identity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein showed 27.3-64 .7 % identity to the bacterial sialyltransferases classified into glycosyltransferase family 80 .
	manualset3
161177	4	411856	7	NULL	NULL	0	NULL	bacterial sialyltransferases	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein showed 27.3-64 .7 % identity to the bacterial sialyltransferases classified into glycosyltransferase family 80 .
	manualset3
161178	5	411856	7	NULL	NULL	0	NULL	glycosyltransferase family 80	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein showed 27.3-64 .7 % identity to the bacterial sialyltransferases classified into glycosyltransferase family 80 .
	manualset3
161179	1	411857	7	NULL	NULL	0	NULL	proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteins can be considered as a microheterogeneous structured media possessing memory and feedback properties .
	manualset3
161180	2	411857	7	NULL	NULL	0	NULL	microheterogeneous structured media	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteins can be considered as a microheterogeneous structured media possessing memory and feedback properties .
	manualset3
161181	3	411857	7	NULL	NULL	0	NULL	memory	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteins can be considered as a microheterogeneous structured media possessing memory and feedback properties .
	manualset3
161182	4	411857	7	NULL	NULL	0	NULL	feedback properties	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteins can be considered as a microheterogeneous structured media possessing memory and feedback properties .
	manualset3
161183	1	411858	7	NULL	NULL	0	NULL	proteolytic cleavage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteolytic cleavage was significantly reduced by the addition of an excess amount of l-arginine ( ) / = 0.2 M ) to the culture medium , which resulted in a marked improvement in the yield of intact hPTH .
	manualset3
161184	2	411858	7	NULL	NULL	NULL	NULL	addition	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proteolytic cleavage was significantly reduced by the addition of an excess amount of l-arginine ( ) / = 0.2 M ) to the culture medium , which resulted in a marked improvement in the yield of intact hPTH .
	manualset3
161186	3	411858	7	NULL	NULL	0	NULL	l-arginine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteolytic cleavage was significantly reduced by the addition of an excess amount of l-arginine ( ) / = 0.2 M ) to the culture medium , which resulted in a marked improvement in the yield of intact hPTH .
	manualset3
161187	4	411858	7	NULL	NULL	0	NULL	0.2 M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteolytic cleavage was significantly reduced by the addition of an excess amount of l-arginine ( ) / = 0.2 M ) to the culture medium , which resulted in a marked improvement in the yield of intact hPTH .
	manualset3
161188	5	411858	7	NULL	NULL	0	NULL	culture medium	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteolytic cleavage was significantly reduced by the addition of an excess amount of l-arginine ( ) / = 0.2 M ) to the culture medium , which resulted in a marked improvement in the yield of intact hPTH .
	manualset3
161189	6	411858	7	NULL	NULL	0	NULL	improvement 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteolytic cleavage was significantly reduced by the addition of an excess amount of l-arginine ( ) / = 0.2 M ) to the culture medium , which resulted in a marked improvement in the yield of intact hPTH .
	manualset3
161190	7	411858	7	NULL	NULL	0	NULL	yield 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteolytic cleavage was significantly reduced by the addition of an excess amount of l-arginine ( ) / = 0.2 M ) to the culture medium , which resulted in a marked improvement in the yield of intact hPTH .
	manualset3
161191	8	411858	7	NULL	NULL	0	NULL	intact hPTH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteolytic cleavage was significantly reduced by the addition of an excess amount of l-arginine ( ) / = 0.2 M ) to the culture medium , which resulted in a marked improvement in the yield of intact hPTH .
	manualset3
169455	9	411858	7	NULL	NULL	0	NULL	excess amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteolytic cleavage was significantly reduced by the addition of an excess amount of l-arginine ( ) / = 0.2 M ) to the culture medium , which resulted in a marked improvement in the yield of intact hPTH .
	manualset3
161192	1	411859	7	NULL	NULL	NULL	NULL	proteomic pattern 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proteomic pattern is consistent with a model of southeast and southwest dispersal and allopatric fragmentation northern of the Amazon Basin , and trans-Amazonian expansion through the Andean Corridor and across the Amazon river between Monte Alegre and Santarm .
	manualset3
161193	2	411859	7	NULL	NULL	0	NULL	 model	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteomic pattern is consistent with a model of southeast and southwest dispersal and allopatric fragmentation northern of the Amazon Basin , and trans-Amazonian expansion through the Andean Corridor and across the Amazon river between Monte Alegre and Santarm .
	manualset3
161194	3	411859	7	NULL	NULL	0	NULL	southeast dispersal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteomic pattern is consistent with a model of southeast and southwest dispersal and allopatric fragmentation northern of the Amazon Basin , and trans-Amazonian expansion through the Andean Corridor and across the Amazon river between Monte Alegre and Santarm .
	manualset3
161195	4	411859	7	NULL	NULL	0	NULL	southwest dispersal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteomic pattern is consistent with a model of southeast and southwest dispersal and allopatric fragmentation northern of the Amazon Basin , and trans-Amazonian expansion through the Andean Corridor and across the Amazon river between Monte Alegre and Santarm .
	manualset3
161196	5	411859	7	NULL	NULL	0	NULL	allopatric fragmentation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteomic pattern is consistent with a model of southeast and southwest dispersal and allopatric fragmentation northern of the Amazon Basin , and trans-Amazonian expansion through the Andean Corridor and across the Amazon river between Monte Alegre and Santarm .
	manualset3
161197	6	411859	7	NULL	NULL	0	NULL	northern of the Amazon Basin	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteomic pattern is consistent with a model of southeast and southwest dispersal and allopatric fragmentation northern of the Amazon Basin , and trans-Amazonian expansion through the Andean Corridor and across the Amazon river between Monte Alegre and Santarm .
	manualset3
161198	7	411859	7	NULL	NULL	0	NULL	trans-Amazonian expansion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteomic pattern is consistent with a model of southeast and southwest dispersal and allopatric fragmentation northern of the Amazon Basin , and trans-Amazonian expansion through the Andean Corridor and across the Amazon river between Monte Alegre and Santarm .
	manualset3
161199	8	411859	7	NULL	NULL	0	NULL	Andean Corridor	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteomic pattern is consistent with a model of southeast and southwest dispersal and allopatric fragmentation northern of the Amazon Basin , and trans-Amazonian expansion through the Andean Corridor and across the Amazon river between Monte Alegre and Santarm .
	manualset3
161200	9	411859	7	NULL	NULL	0	NULL	Amazon river	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteomic pattern is consistent with a model of southeast and southwest dispersal and allopatric fragmentation northern of the Amazon Basin , and trans-Amazonian expansion through the Andean Corridor and across the Amazon river between Monte Alegre and Santarm .
	manualset3
161201	10	411859	7	NULL	NULL	0	NULL	Monte Alegre 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteomic pattern is consistent with a model of southeast and southwest dispersal and allopatric fragmentation northern of the Amazon Basin , and trans-Amazonian expansion through the Andean Corridor and across the Amazon river between Monte Alegre and Santarm .
	manualset3
161202	11	411859	7	NULL	NULL	0	NULL	Santarm	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The proteomic pattern is consistent with a model of southeast and southwest dispersal and allopatric fragmentation northern of the Amazon Basin , and trans-Amazonian expansion through the Andean Corridor and across the Amazon river between Monte Alegre and Santarm .
	manualset3
161203	1	411860	7	NULL	NULL	NULL	NULL	protocol XRT doses	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The protocol XRT doses were 45-50 Gy/20/4 -6 weeks .
	manualset3
161204	2	411860	7	NULL	NULL	0	NULL	 45-50 Gy/20	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The protocol XRT doses were 45-50 Gy/20/4 -6 weeks .
	manualset3
161205	3	411860	7	NULL	NULL	0	NULL	4 -6 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The protocol XRT doses were 45-50 Gy/20/4 -6 weeks .
	manualset3
161206	1	411861	7	NULL	NULL	NULL	NULL	proton transfer parameter	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proton transfer parameter and the coordination number of HNO ( 3 ) and HCl in each cluster have been evaluated , and the wavenumber shifts for the X ( - ) - H ( + ) vibration from the corresponding mode in the isolated molecules have also been predicted .
	manualset3
161207	2	411861	7	NULL	NULL	0	NULL	coordination number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proton transfer parameter and the coordination number of HNO ( 3 ) and HCl in each cluster have been evaluated , and the wavenumber shifts for the X ( - ) - H ( + ) vibration from the corresponding mode in the isolated molecules have also been predicted .
	manualset3
161208	3	411861	7	NULL	NULL	0	NULL	HNO ( 3 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The proton transfer parameter and the coordination number of HNO ( 3 ) and HCl in each cluster have been evaluated , and the wavenumber shifts for the X ( - ) - H ( + ) vibration from the corresponding mode in the isolated molecules have also been predicted .
	manualset3
161209	4	411861	7	NULL	NULL	0	NULL	HCl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The proton transfer parameter and the coordination number of HNO ( 3 ) and HCl in each cluster have been evaluated , and the wavenumber shifts for the X ( - ) - H ( + ) vibration from the corresponding mode in the isolated molecules have also been predicted .
	manualset3
161210	5	411861	7	NULL	NULL	NULL	NULL	cluster	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The proton transfer parameter and the coordination number of HNO ( 3 ) and HCl in each cluster have been evaluated , and the wavenumber shifts for the X ( - ) - H ( + ) vibration from the corresponding mode in the isolated molecules have also been predicted .
	manualset3
161211	6	411861	7	NULL	NULL	0	NULL	wavenumber	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proton transfer parameter and the coordination number of HNO ( 3 ) and HCl in each cluster have been evaluated , and the wavenumber shifts for the X ( - ) - H ( + ) vibration from the corresponding mode in the isolated molecules have also been predicted .
	manualset3
161212	7	411861	7	NULL	NULL	0	NULL	X ( - ) - H ( + ) vibration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The proton transfer parameter and the coordination number of HNO ( 3 ) and HCl in each cluster have been evaluated , and the wavenumber shifts for the X ( - ) - H ( + ) vibration from the corresponding mode in the isolated molecules have also been predicted .
	manualset3
161213	8	411861	7	NULL	NULL	0	NULL	isolated molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The proton transfer parameter and the coordination number of HNO ( 3 ) and HCl in each cluster have been evaluated , and the wavenumber shifts for the X ( - ) - H ( + ) vibration from the corresponding mode in the isolated molecules have also been predicted .
	manualset3
169456	9	411861	7	NULL	NULL	0	NULL	corresponding mode	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The proton transfer parameter and the coordination number of HNO ( 3 ) and HCl in each cluster have been evaluated , and the wavenumber shifts for the X ( - ) - H ( + ) vibration from the corresponding mode in the isolated molecules have also been predicted .
	manualset3
161214	1	411862	7	NULL	NULL	0	NULL	AY19	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	AY19 , a unique mAb was used to better characterize the umbilical cord blood hematopoietic progenitor subpopulations .
	manualset3
161215	2	411862	7	NULL	NULL	0	NULL	mAb	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	AY19 , a unique mAb was used to better characterize the umbilical cord blood hematopoietic progenitor subpopulations .
	manualset3
161216	3	411862	7	NULL	NULL	NULL	NULL	umbilical cord blood hematopoietic progenitor subpopulations	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	AY19 , a unique mAb was used to better characterize the umbilical cord blood hematopoietic progenitor subpopulations .
	manualset3
161217	1	411863	7	NULL	NULL	0	NULL	proximal femur	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The proximal femur is dissected only laterally and only in so far as in necessary to place the DCS .
	manualset3
161219	2	411863	7	NULL	NULL	0	NULL	DCS	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The proximal femur is dissected only laterally and only in so far as in necessary to place the DCS .
	manualset3
161220	1	411864	7	NULL	NULL	0	NULL	psoralen photochemical reaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The psoralen photochemical reaction was chosen for study due to its known specificity for nucleic acids .
	manualset3
161221	2	411864	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The psoralen photochemical reaction was chosen for study due to its known specificity for nucleic acids .
	manualset3
161222	4	411864	7	NULL	NULL	NULL	NULL	nucleic acids	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The psoralen photochemical reaction was chosen for study due to its known specificity for nucleic acids .
	manualset3
162358	3	411864	7	NULL	NULL	0	NULL	specificity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The psoralen photochemical reaction was chosen for study due to its known specificity for nucleic acids .
	manualset3
161223	1	411865	7	NULL	NULL	NULL	NULL	psychology of postponement	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The psychology of postponement ultimately proves to be a psychology of avoidance , growing directly out of the compulsive personality traits of most physicians and their preference for work over family life .
	manualset3
161224	2	411865	7	NULL	NULL	NULL	NULL	psychology of avoidance	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The psychology of postponement ultimately proves to be a psychology of avoidance , growing directly out of the compulsive personality traits of most physicians and their preference for work over family life .
	manualset3
161225	3	411865	7	NULL	NULL	NULL	NULL	personality traits	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The psychology of postponement ultimately proves to be a psychology of avoidance , growing directly out of the compulsive personality traits of most physicians and their preference for work over family life .
	manualset3
161227	4	411865	7	NULL	NULL	NULL	NULL	physicians 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The psychology of postponement ultimately proves to be a psychology of avoidance , growing directly out of the compulsive personality traits of most physicians and their preference for work over family life .
	manualset3
161228	5	411865	7	NULL	NULL	0	NULL	work 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The psychology of postponement ultimately proves to be a psychology of avoidance , growing directly out of the compulsive personality traits of most physicians and their preference for work over family life .
	manualset3
161229	6	411865	7	NULL	NULL	0	NULL	family life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The psychology of postponement ultimately proves to be a psychology of avoidance , growing directly out of the compulsive personality traits of most physicians and their preference for work over family life .
	manualset3
161230	1	411866	7	NULL	NULL	0	NULL	psychosocial orientation	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The psychosocial orientation is female in all of them .
	manualset3
161233	1	411867	7	NULL	NULL	0	NULL	pulmonary AVM	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The pulmonary AVM was removed by segmentectomy of the right lung ( S4 ) .
	manualset3
161234	2	411867	7	NULL	NULL	0	NULL	segmentectomy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The pulmonary AVM was removed by segmentectomy of the right lung ( S4 ) .
	manualset3
161235	3	411867	7	NULL	NULL	0	NULL	right lung ( S4 )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The pulmonary AVM was removed by segmentectomy of the right lung ( S4 ) .
	manualset3
161236	1	411868	7	NULL	NULL	0	NULL	pure polarization state 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The pure polarization state in each segment can be arbitrarily preset .
	manualset3
161237	2	411868	7	NULL	NULL	NULL	NULL	segment 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The pure polarization state in each segment can be arbitrarily preset .
	manualset3
161238	1	411869	7	NULL	NULL	0	NULL	purification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purification of soluble fulvic acids ( FA ) based on a diafiltration technique is carried out on antarctic water and snow samples , characterised by low humic compound content ( 0.1-0 .8 mg/l ) .
	manualset3
161239	2	411869	7	NULL	NULL	0	NULL	soluble fulvic acids ( FA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The purification of soluble fulvic acids ( FA ) based on a diafiltration technique is carried out on antarctic water and snow samples , characterised by low humic compound content ( 0.1-0 .8 mg/l ) .
	manualset3
161240	3	411869	7	NULL	NULL	0	NULL	diafiltration technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purification of soluble fulvic acids ( FA ) based on a diafiltration technique is carried out on antarctic water and snow samples , characterised by low humic compound content ( 0.1-0 .8 mg/l ) .
	manualset3
161241	4	411869	7	NULL	NULL	0	NULL	antarctic water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The purification of soluble fulvic acids ( FA ) based on a diafiltration technique is carried out on antarctic water and snow samples , characterised by low humic compound content ( 0.1-0 .8 mg/l ) .
	manualset3
161242	5	411869	7	NULL	NULL	0	NULL	snow samples	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The purification of soluble fulvic acids ( FA ) based on a diafiltration technique is carried out on antarctic water and snow samples , characterised by low humic compound content ( 0.1-0 .8 mg/l ) .
	manualset3
161243	6	411869	7	NULL	NULL	0	NULL	low humic compound content	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The purification of soluble fulvic acids ( FA ) based on a diafiltration technique is carried out on antarctic water and snow samples , characterised by low humic compound content ( 0.1-0 .8 mg/l ) .
	manualset3
161244	7	411869	7	NULL	NULL	0	NULL	0.1-0 .8 mg/l 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The purification of soluble fulvic acids ( FA ) based on a diafiltration technique is carried out on antarctic water and snow samples , characterised by low humic compound content ( 0.1-0 .8 mg/l ) .
	manualset3
161245	1	411870	7	NULL	NULL	0	NULL	purification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purification of the antigen by ultracentrifugation ( AgU ) was undertaken using 10 ( 9 ) infected cells , and by affinity chromatography ( AgAc ) using 10 ( 7 ) infected cells .
	manualset3
161246	2	411870	7	NULL	NULL	0	NULL	 antigen	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The purification of the antigen by ultracentrifugation ( AgU ) was undertaken using 10 ( 9 ) infected cells , and by affinity chromatography ( AgAc ) using 10 ( 7 ) infected cells .
	manualset3
161247	3	411870	7	NULL	NULL	0	NULL	ultracentrifugation ( AgU )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purification of the antigen by ultracentrifugation ( AgU ) was undertaken using 10 ( 9 ) infected cells , and by affinity chromatography ( AgAc ) using 10 ( 7 ) infected cells .
	manualset3
161248	4	411870	7	NULL	NULL	0	NULL	10 ( 9 ) infected cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The purification of the antigen by ultracentrifugation ( AgU ) was undertaken using 10 ( 9 ) infected cells , and by affinity chromatography ( AgAc ) using 10 ( 7 ) infected cells .
	manualset3
161249	5	411870	7	NULL	NULL	0	NULL	affinity chromatography ( AgAc )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purification of the antigen by ultracentrifugation ( AgU ) was undertaken using 10 ( 9 ) infected cells , and by affinity chromatography ( AgAc ) using 10 ( 7 ) infected cells .
	manualset3
161250	6	411870	7	NULL	NULL	0	NULL	10 ( 7 ) infected cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The purification of the antigen by ultracentrifugation ( AgU ) was undertaken using 10 ( 9 ) infected cells , and by affinity chromatography ( AgAc ) using 10 ( 7 ) infected cells .
	manualset3
161251	1	411871	7	NULL	NULL	0	NULL	 purification procedure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purification procedure entailed ammonium sulphate precipitation , gel filtration and preparative PAGE .
	manualset3
161252	2	411871	7	NULL	NULL	0	NULL	ammonium sulphate precipitation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purification procedure entailed ammonium sulphate precipitation , gel filtration and preparative PAGE .
	manualset3
161253	3	411871	7	NULL	NULL	0	NULL	gel filtration	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purification procedure entailed ammonium sulphate precipitation , gel filtration and preparative PAGE .
	manualset3
161254	4	411871	7	NULL	NULL	0	NULL	preparative PAGE	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purification procedure entailed ammonium sulphate precipitation , gel filtration and preparative PAGE .
	manualset3
161255	1	411872	7	NULL	NULL	0	NULL	A/E	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A/E in patients with inferior AMI ( 1.01 + / - 0.24 , mean + / - standard deviation ) was significantly greater than in those with anterior AMI ( 0.80 + / - 0.16 , p less than 0.001 ) and angina pectoris ( 0.79 + / - 0.17 , p less than 0.01 ) and in normal subjects ( 0.70 + / - 0.17 , p less than 0.001 ) .
	manualset3
161257	2	411872	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A/E in patients with inferior AMI ( 1.01 + / - 0.24 , mean + / - standard deviation ) was significantly greater than in those with anterior AMI ( 0.80 + / - 0.16 , p less than 0.001 ) and angina pectoris ( 0.79 + / - 0.17 , p less than 0.01 ) and in normal subjects ( 0.70 + / - 0.17 , p less than 0.001 ) .
	manualset3
161258	3	411872	7	NULL	NULL	0	NULL	inferior AMI 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A/E in patients with inferior AMI ( 1.01 + / - 0.24 , mean + / - standard deviation ) was significantly greater than in those with anterior AMI ( 0.80 + / - 0.16 , p less than 0.001 ) and angina pectoris ( 0.79 + / - 0.17 , p less than 0.01 ) and in normal subjects ( 0.70 + / - 0.17 , p less than 0.001 ) .
	manualset3
161259	4	411872	7	NULL	NULL	0	NULL	1.01 + / - 0.24 , mean + / - standard deviation	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A/E in patients with inferior AMI ( 1.01 + / - 0.24 , mean + / - standard deviation ) was significantly greater than in those with anterior AMI ( 0.80 + / - 0.16 , p less than 0.001 ) and angina pectoris ( 0.79 + / - 0.17 , p less than 0.01 ) and in normal subjects ( 0.70 + / - 0.17 , p less than 0.001 ) .
	manualset3
161260	5	411872	7	NULL	NULL	0	NULL	anterior AMI	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A/E in patients with inferior AMI ( 1.01 + / - 0.24 , mean + / - standard deviation ) was significantly greater than in those with anterior AMI ( 0.80 + / - 0.16 , p less than 0.001 ) and angina pectoris ( 0.79 + / - 0.17 , p less than 0.01 ) and in normal subjects ( 0.70 + / - 0.17 , p less than 0.001 ) .
	manualset3
161261	6	411872	7	NULL	NULL	0	NULL	 0.80 + / - 0.16 , p less than 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A/E in patients with inferior AMI ( 1.01 + / - 0.24 , mean + / - standard deviation ) was significantly greater than in those with anterior AMI ( 0.80 + / - 0.16 , p less than 0.001 ) and angina pectoris ( 0.79 + / - 0.17 , p less than 0.01 ) and in normal subjects ( 0.70 + / - 0.17 , p less than 0.001 ) .
	manualset3
161262	7	411872	7	NULL	NULL	0	NULL	angina pectoris	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A/E in patients with inferior AMI ( 1.01 + / - 0.24 , mean + / - standard deviation ) was significantly greater than in those with anterior AMI ( 0.80 + / - 0.16 , p less than 0.001 ) and angina pectoris ( 0.79 + / - 0.17 , p less than 0.01 ) and in normal subjects ( 0.70 + / - 0.17 , p less than 0.001 ) .
	manualset3
161263	8	411872	7	NULL	NULL	0	NULL	 0.79 + / - 0.17 , p less than 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A/E in patients with inferior AMI ( 1.01 + / - 0.24 , mean + / - standard deviation ) was significantly greater than in those with anterior AMI ( 0.80 + / - 0.16 , p less than 0.001 ) and angina pectoris ( 0.79 + / - 0.17 , p less than 0.01 ) and in normal subjects ( 0.70 + / - 0.17 , p less than 0.001 ) .
	manualset3
161264	9	411872	7	NULL	NULL	0	NULL	normal subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A/E in patients with inferior AMI ( 1.01 + / - 0.24 , mean + / - standard deviation ) was significantly greater than in those with anterior AMI ( 0.80 + / - 0.16 , p less than 0.001 ) and angina pectoris ( 0.79 + / - 0.17 , p less than 0.01 ) and in normal subjects ( 0.70 + / - 0.17 , p less than 0.001 ) .
	manualset3
161265	10	411872	7	NULL	NULL	0	NULL	 0.70 + / - 0.17 , p less than 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A/E in patients with inferior AMI ( 1.01 + / - 0.24 , mean + / - standard deviation ) was significantly greater than in those with anterior AMI ( 0.80 + / - 0.16 , p less than 0.001 ) and angina pectoris ( 0.79 + / - 0.17 , p less than 0.01 ) and in normal subjects ( 0.70 + / - 0.17 , p less than 0.001 ) .
	manualset3
161266	1	411873	7	NULL	NULL	0	NULL	purification steps	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purification steps included gel filtration , ammonium sulphate precipitation , centrifugal microconcentration and fast-performance liquid chromatography .
	manualset3
161267	2	411873	7	NULL	NULL	0	NULL	gel filtration	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purification steps included gel filtration , ammonium sulphate precipitation , centrifugal microconcentration and fast-performance liquid chromatography .
	manualset3
161268	3	411873	7	NULL	NULL	0	NULL	ammonium sulphate precipitation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purification steps included gel filtration , ammonium sulphate precipitation , centrifugal microconcentration and fast-performance liquid chromatography .
	manualset3
161269	4	411873	7	NULL	NULL	0	NULL	centrifugal microconcentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purification steps included gel filtration , ammonium sulphate precipitation , centrifugal microconcentration and fast-performance liquid chromatography .
	manualset3
161270	5	411873	7	NULL	NULL	0	NULL	fast-performance liquid chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purification steps included gel filtration , ammonium sulphate precipitation , centrifugal microconcentration and fast-performance liquid chromatography .
	manualset3
161271	1	411874	7	NULL	NULL	0	NULL	purified NF-GM2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The purified NF-GM2 consists of 50 ( p50 ) and 65 kDa ( p65 ) polypeptides and has a binding activity specific for both the GM-CSF and immunoglobulin kappa ( GGAAAGTCCC ) enhancers .
	manualset3
161272	2	411874	7	NULL	NULL	0	NULL	50 ( p50 ) polypeptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The purified NF-GM2 consists of 50 ( p50 ) and 65 kDa ( p65 ) polypeptides and has a binding activity specific for both the GM-CSF and immunoglobulin kappa ( GGAAAGTCCC ) enhancers .
	manualset3
161273	3	411874	7	NULL	NULL	0	NULL	65 kDa ( p65 ) polypeptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The purified NF-GM2 consists of 50 ( p50 ) and 65 kDa ( p65 ) polypeptides and has a binding activity specific for both the GM-CSF and immunoglobulin kappa ( GGAAAGTCCC ) enhancers .
	manualset3
161274	4	411874	7	NULL	NULL	0	NULL	activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purified NF-GM2 consists of 50 ( p50 ) and 65 kDa ( p65 ) polypeptides and has a binding activity specific for both the GM-CSF and immunoglobulin kappa ( GGAAAGTCCC ) enhancers .
	manualset3
161275	5	411874	7	NULL	NULL	0	NULL	GM-CSF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The purified NF-GM2 consists of 50 ( p50 ) and 65 kDa ( p65 ) polypeptides and has a binding activity specific for both the GM-CSF and immunoglobulin kappa ( GGAAAGTCCC ) enhancers .
	manualset3
161276	6	411874	7	NULL	NULL	0	NULL	immunoglobulin kappa ( GGAAAGTCCC ) enhancers 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The purified NF-GM2 consists of 50 ( p50 ) and 65 kDa ( p65 ) polypeptides and has a binding activity specific for both the GM-CSF and immunoglobulin kappa ( GGAAAGTCCC ) enhancers .
	manualset3
161277	1	411875	7	NULL	NULL	0	NULL	purified recombinant CCT complexes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The purified recombinant CCT complexes were indistinguishable from the endogenous CCT purified from HeLa cells in terms of morphology and function .
	manualset3
161278	2	411875	7	NULL	NULL	0	NULL	endogenous CCT	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The purified recombinant CCT complexes were indistinguishable from the endogenous CCT purified from HeLa cells in terms of morphology and function .
	manualset3
161279	3	411875	7	NULL	NULL	0	NULL	HeLa cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The purified recombinant CCT complexes were indistinguishable from the endogenous CCT purified from HeLa cells in terms of morphology and function .
	manualset3
161280	4	411875	7	NULL	NULL	0	NULL	morphology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purified recombinant CCT complexes were indistinguishable from the endogenous CCT purified from HeLa cells in terms of morphology and function .
	manualset3
161281	5	411875	7	NULL	NULL	0	NULL	function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purified recombinant CCT complexes were indistinguishable from the endogenous CCT purified from HeLa cells in terms of morphology and function .
	manualset3
161282	1	411876	7	NULL	NULL	NULL	NULL	purine phosphoribosyltransferase activities	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purine phosphoribosyltransferase activities were between two and three orders of magnitude greater than purine de novo synthesis .
	manualset3
161283	2	411876	7	NULL	NULL	0	NULL	two orders of magnitude 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purine phosphoribosyltransferase activities were between two and three orders of magnitude greater than purine de novo synthesis .
	manualset3
161284	3	411876	7	NULL	NULL	0	NULL	three orders of magnitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purine phosphoribosyltransferase activities were between two and three orders of magnitude greater than purine de novo synthesis .
	manualset3
161285	4	411876	7	NULL	NULL	0	NULL	purine de novo synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purine phosphoribosyltransferase activities were between two and three orders of magnitude greater than purine de novo synthesis .
	manualset3
161286	1	411877	7	NULL	NULL	0	NULL	 purpose	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose is to assist busy practitioners , students , researchers , or scholars to stay abreast of these items of progress in obstetrics and gynecology that have recently achieved a substantial degree of authoritative acceptance , whether in their own field of special interest or another .
	manualset3
161287	2	411877	7	NULL	NULL	0	NULL	busy practitioners	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose is to assist busy practitioners , students , researchers , or scholars to stay abreast of these items of progress in obstetrics and gynecology that have recently achieved a substantial degree of authoritative acceptance , whether in their own field of special interest or another .
	manualset3
161288	3	411877	7	NULL	NULL	0	NULL	students	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose is to assist busy practitioners , students , researchers , or scholars to stay abreast of these items of progress in obstetrics and gynecology that have recently achieved a substantial degree of authoritative acceptance , whether in their own field of special interest or another .
	manualset3
161289	4	411877	7	NULL	NULL	0	NULL	researchers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose is to assist busy practitioners , students , researchers , or scholars to stay abreast of these items of progress in obstetrics and gynecology that have recently achieved a substantial degree of authoritative acceptance , whether in their own field of special interest or another .
	manualset3
161290	5	411877	7	NULL	NULL	0	NULL	scholars	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose is to assist busy practitioners , students , researchers , or scholars to stay abreast of these items of progress in obstetrics and gynecology that have recently achieved a substantial degree of authoritative acceptance , whether in their own field of special interest or another .
	manualset3
161291	6	411877	7	NULL	NULL	0	NULL	obstetrics and gynecology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose is to assist busy practitioners , students , researchers , or scholars to stay abreast of these items of progress in obstetrics and gynecology that have recently achieved a substantial degree of authoritative acceptance , whether in their own field of special interest or another .
	manualset3
161292	7	411877	7	NULL	NULL	NULL	NULL	degree	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose is to assist busy practitioners , students , researchers , or scholars to stay abreast of these items of progress in obstetrics and gynecology that have recently achieved a substantial degree of authoritative acceptance , whether in their own field of special interest or another .
	manualset3
161293	8	411877	7	NULL	NULL	NULL	NULL	acceptance	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose is to assist busy practitioners , students , researchers , or scholars to stay abreast of these items of progress in obstetrics and gynecology that have recently achieved a substantial degree of authoritative acceptance , whether in their own field of special interest or another .
	manualset3
161294	9	411877	7	NULL	NULL	0	NULL	field 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose is to assist busy practitioners , students , researchers , or scholars to stay abreast of these items of progress in obstetrics and gynecology that have recently achieved a substantial degree of authoritative acceptance , whether in their own field of special interest or another .
	manualset3
161296	10	411877	7	NULL	NULL	0	NULL	 progress	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose is to assist busy practitioners , students , researchers , or scholars to stay abreast of these items of progress in obstetrics and gynecology that have recently achieved a substantial degree of authoritative acceptance , whether in their own field of special interest or another .
	manualset3
169457	11	411877	7	NULL	NULL	0	NULL	special interest	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose is to assist busy practitioners , students , researchers , or scholars to stay abreast of these items of progress in obstetrics and gynecology that have recently achieved a substantial degree of authoritative acceptance , whether in their own field of special interest or another .
	manualset3
161297	1	411878	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of our research was to evaluate the attitude to face the life cycle and the impact that the experience of childhood leukemia may have had in a group of adolescents who had the disease cured .
	manualset3
161298	2	411878	7	NULL	NULL	0	NULL	research 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of our research was to evaluate the attitude to face the life cycle and the impact that the experience of childhood leukemia may have had in a group of adolescents who had the disease cured .
	manualset3
161299	3	411878	7	NULL	NULL	0	NULL	attitude	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of our research was to evaluate the attitude to face the life cycle and the impact that the experience of childhood leukemia may have had in a group of adolescents who had the disease cured .
	manualset3
161300	4	411878	7	NULL	NULL	0	NULL	 life cycle	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of our research was to evaluate the attitude to face the life cycle and the impact that the experience of childhood leukemia may have had in a group of adolescents who had the disease cured .
	manualset3
161301	5	411878	7	NULL	NULL	0	NULL	impact 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of our research was to evaluate the attitude to face the life cycle and the impact that the experience of childhood leukemia may have had in a group of adolescents who had the disease cured .
	manualset3
161302	6	411878	7	NULL	NULL	0	NULL	experience 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of our research was to evaluate the attitude to face the life cycle and the impact that the experience of childhood leukemia may have had in a group of adolescents who had the disease cured .
	manualset3
161303	7	411878	7	NULL	NULL	0	NULL	childhood leukemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of our research was to evaluate the attitude to face the life cycle and the impact that the experience of childhood leukemia may have had in a group of adolescents who had the disease cured .
	manualset3
161304	8	411878	7	NULL	NULL	0	NULL	group of adolescents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of our research was to evaluate the attitude to face the life cycle and the impact that the experience of childhood leukemia may have had in a group of adolescents who had the disease cured .
	manualset3
161305	9	411878	7	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of our research was to evaluate the attitude to face the life cycle and the impact that the experience of childhood leukemia may have had in a group of adolescents who had the disease cured .
	manualset3
161306	1	411879	7	NULL	NULL	0	NULL	purpose 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of our study was to find out the intensity of free radical reactions in pediatric patients with different forms of juvenile chronic arthritis ( JCA ) on the basis of carbonyl groups ' content in plasma proteins , evaluated with the use of Levine 's method .
	manualset3
161308	2	411879	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of our study was to find out the intensity of free radical reactions in pediatric patients with different forms of juvenile chronic arthritis ( JCA ) on the basis of carbonyl groups ' content in plasma proteins , evaluated with the use of Levine 's method .
	manualset3
161309	3	411879	7	NULL	NULL	0	NULL	intensity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of our study was to find out the intensity of free radical reactions in pediatric patients with different forms of juvenile chronic arthritis ( JCA ) on the basis of carbonyl groups ' content in plasma proteins , evaluated with the use of Levine 's method .
	manualset3
161310	4	411879	7	NULL	NULL	0	NULL	free radical reactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of our study was to find out the intensity of free radical reactions in pediatric patients with different forms of juvenile chronic arthritis ( JCA ) on the basis of carbonyl groups ' content in plasma proteins , evaluated with the use of Levine 's method .
	manualset3
161311	5	411879	7	NULL	NULL	0	NULL	pediatric patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of our study was to find out the intensity of free radical reactions in pediatric patients with different forms of juvenile chronic arthritis ( JCA ) on the basis of carbonyl groups ' content in plasma proteins , evaluated with the use of Levine 's method .
	manualset3
161312	6	411879	7	NULL	NULL	0	NULL	juvenile chronic arthritis ( JCA )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of our study was to find out the intensity of free radical reactions in pediatric patients with different forms of juvenile chronic arthritis ( JCA ) on the basis of carbonyl groups ' content in plasma proteins , evaluated with the use of Levine 's method .
	manualset3
161313	7	411879	7	NULL	NULL	0	NULL	carbonyl groups ' content	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of our study was to find out the intensity of free radical reactions in pediatric patients with different forms of juvenile chronic arthritis ( JCA ) on the basis of carbonyl groups ' content in plasma proteins , evaluated with the use of Levine 's method .
	manualset3
161314	8	411879	7	NULL	NULL	0	NULL	plasma proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of our study was to find out the intensity of free radical reactions in pediatric patients with different forms of juvenile chronic arthritis ( JCA ) on the basis of carbonyl groups ' content in plasma proteins , evaluated with the use of Levine 's method .
	manualset3
161315	9	411879	7	NULL	NULL	0	NULL	Levine 's method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of our study was to find out the intensity of free radical reactions in pediatric patients with different forms of juvenile chronic arthritis ( JCA ) on the basis of carbonyl groups ' content in plasma proteins , evaluated with the use of Levine 's method .
	manualset3
161316	1	411880	7	NULL	NULL	0	NULL	 purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of our study was to generate a mouse line with A30P knock-in point mutation in SNCA gene and to test if a single point-mutation is able to turn otherwise normal SNCA into a toxic form .
	manualset3
161317	2	411880	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of our study was to generate a mouse line with A30P knock-in point mutation in SNCA gene and to test if a single point-mutation is able to turn otherwise normal SNCA into a toxic form .
	manualset3
161318	3	411880	7	NULL	NULL	0	NULL	mouse line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of our study was to generate a mouse line with A30P knock-in point mutation in SNCA gene and to test if a single point-mutation is able to turn otherwise normal SNCA into a toxic form .
	manualset3
161319	4	411880	7	NULL	NULL	0	NULL	A30P knock-in point mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of our study was to generate a mouse line with A30P knock-in point mutation in SNCA gene and to test if a single point-mutation is able to turn otherwise normal SNCA into a toxic form .
	manualset3
161320	5	411880	7	NULL	NULL	0	NULL	SNCA gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of our study was to generate a mouse line with A30P knock-in point mutation in SNCA gene and to test if a single point-mutation is able to turn otherwise normal SNCA into a toxic form .
	manualset3
161321	6	411880	7	NULL	NULL	0	NULL	single point-mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of our study was to generate a mouse line with A30P knock-in point mutation in SNCA gene and to test if a single point-mutation is able to turn otherwise normal SNCA into a toxic form .
	manualset3
161322	7	411880	7	NULL	NULL	0	NULL	normal SNCA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of our study was to generate a mouse line with A30P knock-in point mutation in SNCA gene and to test if a single point-mutation is able to turn otherwise normal SNCA into a toxic form .
	manualset3
161323	8	411880	7	NULL	NULL	0	NULL	toxic form	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of our study was to generate a mouse line with A30P knock-in point mutation in SNCA gene and to test if a single point-mutation is able to turn otherwise normal SNCA into a toxic form .
	manualset3
161324	1	411881	7	NULL	NULL	0	NULL	 purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the current study was to identify the relationships between competitive performance and tether forces according to distance swam , in the four strokes , and to analyze if relative values of force production are better determinants of swimming performance than absolute values .
	manualset3
161325	2	411881	7	NULL	NULL	0	NULL	current study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the current study was to identify the relationships between competitive performance and tether forces according to distance swam , in the four strokes , and to analyze if relative values of force production are better determinants of swimming performance than absolute values .
	manualset3
161326	3	411881	7	NULL	NULL	0	NULL	relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the current study was to identify the relationships between competitive performance and tether forces according to distance swam , in the four strokes , and to analyze if relative values of force production are better determinants of swimming performance than absolute values .
	manualset3
161327	4	411881	7	NULL	NULL	0	NULL	competitive performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the current study was to identify the relationships between competitive performance and tether forces according to distance swam , in the four strokes , and to analyze if relative values of force production are better determinants of swimming performance than absolute values .
	manualset3
161328	5	411881	7	NULL	NULL	0	NULL	tether	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the current study was to identify the relationships between competitive performance and tether forces according to distance swam , in the four strokes , and to analyze if relative values of force production are better determinants of swimming performance than absolute values .
	manualset3
161329	6	411881	7	NULL	NULL	0	NULL	forces	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the current study was to identify the relationships between competitive performance and tether forces according to distance swam , in the four strokes , and to analyze if relative values of force production are better determinants of swimming performance than absolute values .
	manualset3
161330	7	411881	7	NULL	NULL	NULL	NULL	four strokes	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose of the current study was to identify the relationships between competitive performance and tether forces according to distance swam , in the four strokes , and to analyze if relative values of force production are better determinants of swimming performance than absolute values .
	manualset3
161331	8	411881	7	NULL	NULL	NULL	NULL	relative values 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose of the current study was to identify the relationships between competitive performance and tether forces according to distance swam , in the four strokes , and to analyze if relative values of force production are better determinants of swimming performance than absolute values .
	manualset3
161332	9	411881	7	NULL	NULL	0	NULL	force production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the current study was to identify the relationships between competitive performance and tether forces according to distance swam , in the four strokes , and to analyze if relative values of force production are better determinants of swimming performance than absolute values .
	manualset3
161333	10	411881	7	NULL	NULL	0	NULL	determinants	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the current study was to identify the relationships between competitive performance and tether forces according to distance swam , in the four strokes , and to analyze if relative values of force production are better determinants of swimming performance than absolute values .
	manualset3
161334	11	411881	7	NULL	NULL	0	NULL	swimming performance	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the current study was to identify the relationships between competitive performance and tether forces according to distance swam , in the four strokes , and to analyze if relative values of force production are better determinants of swimming performance than absolute values .
	manualset3
161335	12	411881	7	NULL	NULL	0	NULL	absolute values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the current study was to identify the relationships between competitive performance and tether forces according to distance swam , in the four strokes , and to analyze if relative values of force production are better determinants of swimming performance than absolute values .
	manualset3
161336	1	411882	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the investigation was to assess whether there were psychosocial problems for albinos with white skin and hair .
	manualset3
161337	2	411882	7	NULL	NULL	0	NULL	investigation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the investigation was to assess whether there were psychosocial problems for albinos with white skin and hair .
	manualset3
161338	3	411882	7	NULL	NULL	0	NULL	psychosocial problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the investigation was to assess whether there were psychosocial problems for albinos with white skin and hair .
	manualset3
161339	4	411882	7	NULL	NULL	0	NULL	 albinos	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the investigation was to assess whether there were psychosocial problems for albinos with white skin and hair .
	manualset3
161340	5	411882	7	NULL	NULL	0	NULL	white skin	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the investigation was to assess whether there were psychosocial problems for albinos with white skin and hair .
	manualset3
161341	6	411882	7	NULL	NULL	0	NULL	white hair	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the investigation was to assess whether there were psychosocial problems for albinos with white skin and hair .
	manualset3
161342	1	411883	7	NULL	NULL	0	NULL	Abasic sites	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Abasic sites representing a major class of DNA damage can be quantitated by an ELISA-like assay using an aldehyde reactive probe ( ARP ) .
	manualset3
161343	2	411883	7	NULL	NULL	0	NULL	DNA damage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Abasic sites representing a major class of DNA damage can be quantitated by an ELISA-like assay using an aldehyde reactive probe ( ARP ) .
	manualset3
161344	3	411883	7	NULL	NULL	0	NULL	ELISA-like assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Abasic sites representing a major class of DNA damage can be quantitated by an ELISA-like assay using an aldehyde reactive probe ( ARP ) .
	manualset3
161345	4	411883	7	NULL	NULL	0	NULL	aldehyde reactive probe ( ARP )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Abasic sites representing a major class of DNA damage can be quantitated by an ELISA-like assay using an aldehyde reactive probe ( ARP ) .
	manualset3
161346	1	411884	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the present experiment was to further clarify the involvement of Egr-1 in lens epithelial cell death induced by selenite .
	manualset3
161347	2	411884	7	NULL	NULL	0	NULL	experiment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the present experiment was to further clarify the involvement of Egr-1 in lens epithelial cell death induced by selenite .
	manualset3
161348	3	411884	7	NULL	NULL	0	NULL	involvement	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the present experiment was to further clarify the involvement of Egr-1 in lens epithelial cell death induced by selenite .
	manualset3
161349	4	411884	7	NULL	NULL	0	NULL	Egr-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the present experiment was to further clarify the involvement of Egr-1 in lens epithelial cell death induced by selenite .
	manualset3
161350	5	411884	7	NULL	NULL	NULL	NULL	lens epithelial cell death	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose of the present experiment was to further clarify the involvement of Egr-1 in lens epithelial cell death induced by selenite .
	manualset3
161351	6	411884	7	NULL	NULL	0	NULL	selenite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the present experiment was to further clarify the involvement of Egr-1 in lens epithelial cell death induced by selenite .
	manualset3
161352	1	411885	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the present study was to evaluate the utility of lower thoracic spinal cord stimulation ( SCS ) to activate the expiratory muscles .
	manualset3
161353	2	411885	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the present study was to evaluate the utility of lower thoracic spinal cord stimulation ( SCS ) to activate the expiratory muscles .
	manualset3
161354	3	411885	7	NULL	NULL	0	NULL	utility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the present study was to evaluate the utility of lower thoracic spinal cord stimulation ( SCS ) to activate the expiratory muscles .
	manualset3
161355	4	411885	7	NULL	NULL	0	NULL	lower thoracic spinal cord stimulation ( SCS ) 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the present study was to evaluate the utility of lower thoracic spinal cord stimulation ( SCS ) to activate the expiratory muscles .
	manualset3
161356	5	411885	7	NULL	NULL	0	NULL	expiratory muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the present study was to evaluate the utility of lower thoracic spinal cord stimulation ( SCS ) to activate the expiratory muscles .
	manualset3
161357	1	411886	7	NULL	NULL	0	NULL	 purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the present work was to investigate the participation of estradiol receptors ( ER ) in estrogen-induced axon growth in vitro .
	manualset3
161358	2	411886	7	NULL	NULL	0	NULL	work	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the present work was to investigate the participation of estradiol receptors ( ER ) in estrogen-induced axon growth in vitro .
	manualset3
161359	3	411886	7	NULL	NULL	0	NULL	participation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the present work was to investigate the participation of estradiol receptors ( ER ) in estrogen-induced axon growth in vitro .
	manualset3
161360	4	411886	7	NULL	NULL	0	NULL	estradiol receptors ( ER )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the present work was to investigate the participation of estradiol receptors ( ER ) in estrogen-induced axon growth in vitro .
	manualset3
161361	5	411886	7	NULL	NULL	0	NULL	estrogen-induced axon growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the present work was to investigate the participation of estradiol receptors ( ER ) in estrogen-induced axon growth in vitro .
	manualset3
161362	1	411887	7	NULL	NULL	0	NULL	 purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study is to determine the effect on dental decay , gingival inflammation and oral hygiene of removing dental plaque through supervised daily toothbrushing and flossing in school during a three-year period .
	manualset3
161363	2	411887	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study is to determine the effect on dental decay , gingival inflammation and oral hygiene of removing dental plaque through supervised daily toothbrushing and flossing in school during a three-year period .
	manualset3
161364	3	411887	7	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study is to determine the effect on dental decay , gingival inflammation and oral hygiene of removing dental plaque through supervised daily toothbrushing and flossing in school during a three-year period .
	manualset3
161365	4	411887	7	NULL	NULL	0	NULL	dental decay	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study is to determine the effect on dental decay , gingival inflammation and oral hygiene of removing dental plaque through supervised daily toothbrushing and flossing in school during a three-year period .
	manualset3
161366	5	411887	7	NULL	NULL	0	NULL	gingival inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study is to determine the effect on dental decay , gingival inflammation and oral hygiene of removing dental plaque through supervised daily toothbrushing and flossing in school during a three-year period .
	manualset3
161367	6	411887	7	NULL	NULL	0	NULL	oral hygiene of removing dental plaque	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study is to determine the effect on dental decay , gingival inflammation and oral hygiene of removing dental plaque through supervised daily toothbrushing and flossing in school during a three-year period .
	manualset3
161368	7	411887	7	NULL	NULL	0	NULL	daily toothbrushing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study is to determine the effect on dental decay , gingival inflammation and oral hygiene of removing dental plaque through supervised daily toothbrushing and flossing in school during a three-year period .
	manualset3
161369	8	411887	7	NULL	NULL	0	NULL	 flossing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study is to determine the effect on dental decay , gingival inflammation and oral hygiene of removing dental plaque through supervised daily toothbrushing and flossing in school during a three-year period .
	manualset3
161370	9	411887	7	NULL	NULL	0	NULL	school	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study is to determine the effect on dental decay , gingival inflammation and oral hygiene of removing dental plaque through supervised daily toothbrushing and flossing in school during a three-year period .
	manualset3
161371	10	411887	7	NULL	NULL	0	NULL	three-year period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study is to determine the effect on dental decay , gingival inflammation and oral hygiene of removing dental plaque through supervised daily toothbrushing and flossing in school during a three-year period .
	manualset3
161372	1	411888	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study presented here was to confirm the high yield of group B streptococci ( GBS ) on Granada medium for the detection of pregnant GBS carriers and to compare the results with those obtained using standard Columbia blood agar at two participating centers in Belgium .
	manualset3
161373	2	411888	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study presented here was to confirm the high yield of group B streptococci ( GBS ) on Granada medium for the detection of pregnant GBS carriers and to compare the results with those obtained using standard Columbia blood agar at two participating centers in Belgium .
	manualset3
161374	3	411888	7	NULL	NULL	0	NULL	high yield 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study presented here was to confirm the high yield of group B streptococci ( GBS ) on Granada medium for the detection of pregnant GBS carriers and to compare the results with those obtained using standard Columbia blood agar at two participating centers in Belgium .
	manualset3
161375	4	411888	7	NULL	NULL	0	NULL	group B streptococci ( GBS )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study presented here was to confirm the high yield of group B streptococci ( GBS ) on Granada medium for the detection of pregnant GBS carriers and to compare the results with those obtained using standard Columbia blood agar at two participating centers in Belgium .
	manualset3
161376	5	411888	7	NULL	NULL	0	NULL	 Granada medium	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study presented here was to confirm the high yield of group B streptococci ( GBS ) on Granada medium for the detection of pregnant GBS carriers and to compare the results with those obtained using standard Columbia blood agar at two participating centers in Belgium .
	manualset3
161377	6	411888	7	NULL	NULL	0	NULL	pregnant GBS carriers	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study presented here was to confirm the high yield of group B streptococci ( GBS ) on Granada medium for the detection of pregnant GBS carriers and to compare the results with those obtained using standard Columbia blood agar at two participating centers in Belgium .
	manualset3
161378	7	411888	7	NULL	NULL	0	NULL	results	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study presented here was to confirm the high yield of group B streptococci ( GBS ) on Granada medium for the detection of pregnant GBS carriers and to compare the results with those obtained using standard Columbia blood agar at two participating centers in Belgium .
	manualset3
161379	8	411888	7	NULL	NULL	0	NULL	standard Columbia blood agar	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study presented here was to confirm the high yield of group B streptococci ( GBS ) on Granada medium for the detection of pregnant GBS carriers and to compare the results with those obtained using standard Columbia blood agar at two participating centers in Belgium .
	manualset3
161380	9	411888	7	NULL	NULL	0	NULL	Belgium	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study presented here was to confirm the high yield of group B streptococci ( GBS ) on Granada medium for the detection of pregnant GBS carriers and to compare the results with those obtained using standard Columbia blood agar at two participating centers in Belgium .
	manualset3
161381	10	411888	7	NULL	NULL	0	NULL	detection 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study presented here was to confirm the high yield of group B streptococci ( GBS ) on Granada medium for the detection of pregnant GBS carriers and to compare the results with those obtained using standard Columbia blood agar at two participating centers in Belgium .
	manualset3
162507	11	411888	7	NULL	NULL	0	NULL	two participating centers	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study presented here was to confirm the high yield of group B streptococci ( GBS ) on Granada medium for the detection of pregnant GBS carriers and to compare the results with those obtained using standard Columbia blood agar at two participating centers in Belgium .
	manualset3
161382	1	411889	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study was to describe the presentation and management of urinary incontinence because of severe labial adhesions .
	manualset3
161383	2	411889	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study was to describe the presentation and management of urinary incontinence because of severe labial adhesions .
	manualset3
161384	3	411889	7	NULL	NULL	NULL	NULL	presentation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose of the study was to describe the presentation and management of urinary incontinence because of severe labial adhesions .
	manualset3
161385	4	411889	7	NULL	NULL	NULL	NULL	management	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose of the study was to describe the presentation and management of urinary incontinence because of severe labial adhesions .
	manualset3
161386	5	411889	7	NULL	NULL	0	NULL	urinary incontinence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study was to describe the presentation and management of urinary incontinence because of severe labial adhesions .
	manualset3
161387	6	411889	7	NULL	NULL	0	NULL	labial adhesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study was to describe the presentation and management of urinary incontinence because of severe labial adhesions .
	manualset3
161388	1	411890	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study was to determine clinical and diagnostic distinctions between the episodes of recurrent depression and bipolar depression .
	manualset3
161389	2	411890	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study was to determine clinical and diagnostic distinctions between the episodes of recurrent depression and bipolar depression .
	manualset3
161390	3	411890	7	NULL	NULL	0	NULL	clinical distinction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study was to determine clinical and diagnostic distinctions between the episodes of recurrent depression and bipolar depression .
	manualset3
161391	4	411890	7	NULL	NULL	0	NULL	diagnostic distinctions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study was to determine clinical and diagnostic distinctions between the episodes of recurrent depression and bipolar depression .
	manualset3
161392	5	411890	7	NULL	NULL	0	NULL	episodes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study was to determine clinical and diagnostic distinctions between the episodes of recurrent depression and bipolar depression .
	manualset3
161393	6	411890	7	NULL	NULL	0	NULL	recurrent depression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study was to determine clinical and diagnostic distinctions between the episodes of recurrent depression and bipolar depression .
	manualset3
161394	7	411890	7	NULL	NULL	0	NULL	bipolar depression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study was to determine clinical and diagnostic distinctions between the episodes of recurrent depression and bipolar depression .
	manualset3
161395	1	411891	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study was to investigate the effect of polarizing mixture on the level of lactic and pyruvic acids in blood and cerebro-spinal fluid of patients with acute ischaemic stroke in the earliest phase of illness .
	manualset3
161396	2	411891	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study was to investigate the effect of polarizing mixture on the level of lactic and pyruvic acids in blood and cerebro-spinal fluid of patients with acute ischaemic stroke in the earliest phase of illness .
	manualset3
161397	3	411891	7	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study was to investigate the effect of polarizing mixture on the level of lactic and pyruvic acids in blood and cerebro-spinal fluid of patients with acute ischaemic stroke in the earliest phase of illness .
	manualset3
161398	4	411891	7	NULL	NULL	0	NULL	polarizing mixture	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study was to investigate the effect of polarizing mixture on the level of lactic and pyruvic acids in blood and cerebro-spinal fluid of patients with acute ischaemic stroke in the earliest phase of illness .
	manualset3
161399	5	411891	7	NULL	NULL	NULL	NULL	level of lactic acid	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose of the study was to investigate the effect of polarizing mixture on the level of lactic and pyruvic acids in blood and cerebro-spinal fluid of patients with acute ischaemic stroke in the earliest phase of illness .
	manualset3
161400	6	411891	7	NULL	NULL	0	NULL	level of pyruvic acids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study was to investigate the effect of polarizing mixture on the level of lactic and pyruvic acids in blood and cerebro-spinal fluid of patients with acute ischaemic stroke in the earliest phase of illness .
	manualset3
161401	7	411891	7	NULL	NULL	NULL	NULL	blood 	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose of the study was to investigate the effect of polarizing mixture on the level of lactic and pyruvic acids in blood and cerebro-spinal fluid of patients with acute ischaemic stroke in the earliest phase of illness .
	manualset3
161402	8	411891	7	NULL	NULL	0	NULL	cerebro-spinal fluid	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study was to investigate the effect of polarizing mixture on the level of lactic and pyruvic acids in blood and cerebro-spinal fluid of patients with acute ischaemic stroke in the earliest phase of illness .
	manualset3
161403	9	411891	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study was to investigate the effect of polarizing mixture on the level of lactic and pyruvic acids in blood and cerebro-spinal fluid of patients with acute ischaemic stroke in the earliest phase of illness .
	manualset3
161404	10	411891	7	NULL	NULL	0	NULL	acute ischaemic stroke	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study was to investigate the effect of polarizing mixture on the level of lactic and pyruvic acids in blood and cerebro-spinal fluid of patients with acute ischaemic stroke in the earliest phase of illness .
	manualset3
161405	11	411891	7	NULL	NULL	0	NULL	 earliest phase	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study was to investigate the effect of polarizing mixture on the level of lactic and pyruvic acids in blood and cerebro-spinal fluid of patients with acute ischaemic stroke in the earliest phase of illness .
	manualset3
161406	12	411891	7	NULL	NULL	0	NULL	illness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the study was to investigate the effect of polarizing mixture on the level of lactic and pyruvic acids in blood and cerebro-spinal fluid of patients with acute ischaemic stroke in the earliest phase of illness .
	manualset3
161407	1	411892	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the vertebral column resection was to eliminate pain , prevent progressive deformity , and obtain the maximum correction necessary to achieve spinal balance in the coronal and sagittal plane .
	manualset3
161408	2	411892	7	NULL	NULL	0	NULL	vertebral column resection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the vertebral column resection was to eliminate pain , prevent progressive deformity , and obtain the maximum correction necessary to achieve spinal balance in the coronal and sagittal plane .
	manualset3
161409	3	411892	7	NULL	NULL	0	NULL	pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the vertebral column resection was to eliminate pain , prevent progressive deformity , and obtain the maximum correction necessary to achieve spinal balance in the coronal and sagittal plane .
	manualset3
161410	4	411892	7	NULL	NULL	0	NULL	progressive deformity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the vertebral column resection was to eliminate pain , prevent progressive deformity , and obtain the maximum correction necessary to achieve spinal balance in the coronal and sagittal plane .
	manualset3
161411	5	411892	7	NULL	NULL	0	NULL	 maximum correction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the vertebral column resection was to eliminate pain , prevent progressive deformity , and obtain the maximum correction necessary to achieve spinal balance in the coronal and sagittal plane .
	manualset3
161412	6	411892	7	NULL	NULL	0	NULL	spinal balance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the vertebral column resection was to eliminate pain , prevent progressive deformity , and obtain the maximum correction necessary to achieve spinal balance in the coronal and sagittal plane .
	manualset3
161413	7	411892	7	NULL	NULL	0	NULL	coronal plane .	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the vertebral column resection was to eliminate pain , prevent progressive deformity , and obtain the maximum correction necessary to achieve spinal balance in the coronal and sagittal plane .
	manualset3
161414	8	411892	7	NULL	NULL	0	NULL	sagittal plane 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the vertebral column resection was to eliminate pain , prevent progressive deformity , and obtain the maximum correction necessary to achieve spinal balance in the coronal and sagittal plane .
	manualset3
161415	1	411893	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this article is to identify four herbs that consumers commonly select for the treatment of hypertension and identify nursing care considerations for their use .
	manualset3
161416	2	411893	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this article is to identify four herbs that consumers commonly select for the treatment of hypertension and identify nursing care considerations for their use .
	manualset3
161417	3	411893	7	NULL	NULL	0	NULL	four herbs	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this article is to identify four herbs that consumers commonly select for the treatment of hypertension and identify nursing care considerations for their use .
	manualset3
161418	4	411893	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this article is to identify four herbs that consumers commonly select for the treatment of hypertension and identify nursing care considerations for their use .
	manualset3
161419	5	411893	7	NULL	NULL	0	NULL	hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this article is to identify four herbs that consumers commonly select for the treatment of hypertension and identify nursing care considerations for their use .
	manualset3
161420	6	411893	7	NULL	NULL	0	NULL	nursing care	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this article is to identify four herbs that consumers commonly select for the treatment of hypertension and identify nursing care considerations for their use .
	manualset3
162360	7	411893	7	NULL	NULL	0	NULL	consumers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this article is to identify four herbs that consumers commonly select for the treatment of hypertension and identify nursing care considerations for their use .
	manualset3
161421	1	411894	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this article is to review the literature on the reliability and validity of scores for Waddell 's nonorganic signs , descriptions of pain behavior and symptom magnification , coefficients of variation , correlations between musculoskeletal evaluation and function , grip measurements , and the relationship between heart rate and pain intensity .
	manualset3
161422	2	411894	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this article is to review the literature on the reliability and validity of scores for Waddell 's nonorganic signs , descriptions of pain behavior and symptom magnification , coefficients of variation , correlations between musculoskeletal evaluation and function , grip measurements , and the relationship between heart rate and pain intensity .
	manualset3
161423	3	411894	7	NULL	NULL	0	NULL	literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this article is to review the literature on the reliability and validity of scores for Waddell 's nonorganic signs , descriptions of pain behavior and symptom magnification , coefficients of variation , correlations between musculoskeletal evaluation and function , grip measurements , and the relationship between heart rate and pain intensity .
	manualset3
161424	4	411894	7	NULL	NULL	NULL	NULL	 scores	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose of this article is to review the literature on the reliability and validity of scores for Waddell 's nonorganic signs , descriptions of pain behavior and symptom magnification , coefficients of variation , correlations between musculoskeletal evaluation and function , grip measurements , and the relationship between heart rate and pain intensity .
	manualset3
161425	5	411894	7	NULL	NULL	NULL	NULL	Waddell 's nonorganic signs	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose of this article is to review the literature on the reliability and validity of scores for Waddell 's nonorganic signs , descriptions of pain behavior and symptom magnification , coefficients of variation , correlations between musculoskeletal evaluation and function , grip measurements , and the relationship between heart rate and pain intensity .
	manualset3
161426	6	411894	7	NULL	NULL	NULL	NULL	descriptions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose of this article is to review the literature on the reliability and validity of scores for Waddell 's nonorganic signs , descriptions of pain behavior and symptom magnification , coefficients of variation , correlations between musculoskeletal evaluation and function , grip measurements , and the relationship between heart rate and pain intensity .
	manualset3
161427	7	411894	7	NULL	NULL	0	NULL	pain behavior	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this article is to review the literature on the reliability and validity of scores for Waddell 's nonorganic signs , descriptions of pain behavior and symptom magnification , coefficients of variation , correlations between musculoskeletal evaluation and function , grip measurements , and the relationship between heart rate and pain intensity .
	manualset3
161428	8	411894	7	NULL	NULL	0	NULL	symptom magnification	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this article is to review the literature on the reliability and validity of scores for Waddell 's nonorganic signs , descriptions of pain behavior and symptom magnification , coefficients of variation , correlations between musculoskeletal evaluation and function , grip measurements , and the relationship between heart rate and pain intensity .
	manualset3
161429	9	411894	7	NULL	NULL	0	NULL	coefficients of variation	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this article is to review the literature on the reliability and validity of scores for Waddell 's nonorganic signs , descriptions of pain behavior and symptom magnification , coefficients of variation , correlations between musculoskeletal evaluation and function , grip measurements , and the relationship between heart rate and pain intensity .
	manualset3
161430	10	411894	7	NULL	NULL	0	NULL	musculoskeletal evaluation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this article is to review the literature on the reliability and validity of scores for Waddell 's nonorganic signs , descriptions of pain behavior and symptom magnification , coefficients of variation , correlations between musculoskeletal evaluation and function , grip measurements , and the relationship between heart rate and pain intensity .
	manualset3
161431	11	411894	7	NULL	NULL	0	NULL	function measurement	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this article is to review the literature on the reliability and validity of scores for Waddell 's nonorganic signs , descriptions of pain behavior and symptom magnification , coefficients of variation , correlations between musculoskeletal evaluation and function , grip measurements , and the relationship between heart rate and pain intensity .
	manualset3
161432	12	411894	7	NULL	NULL	NULL	NULL	grip measurements 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose of this article is to review the literature on the reliability and validity of scores for Waddell 's nonorganic signs , descriptions of pain behavior and symptom magnification , coefficients of variation , correlations between musculoskeletal evaluation and function , grip measurements , and the relationship between heart rate and pain intensity .
	manualset3
161433	13	411894	7	NULL	NULL	0	NULL	 relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this article is to review the literature on the reliability and validity of scores for Waddell 's nonorganic signs , descriptions of pain behavior and symptom magnification , coefficients of variation , correlations between musculoskeletal evaluation and function , grip measurements , and the relationship between heart rate and pain intensity .
	manualset3
161434	14	411894	7	NULL	NULL	0	NULL	heart rate 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this article is to review the literature on the reliability and validity of scores for Waddell 's nonorganic signs , descriptions of pain behavior and symptom magnification , coefficients of variation , correlations between musculoskeletal evaluation and function , grip measurements , and the relationship between heart rate and pain intensity .
	manualset3
161435	15	411894	7	NULL	NULL	0	NULL	pain intensity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this article is to review the literature on the reliability and validity of scores for Waddell 's nonorganic signs , descriptions of pain behavior and symptom magnification , coefficients of variation , correlations between musculoskeletal evaluation and function , grip measurements , and the relationship between heart rate and pain intensity .
	manualset3
161436	16	411894	7	NULL	NULL	0	NULL	correlations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this article is to review the literature on the reliability and validity of scores for Waddell 's nonorganic signs , descriptions of pain behavior and symptom magnification , coefficients of variation , correlations between musculoskeletal evaluation and function , grip measurements , and the relationship between heart rate and pain intensity .
	manualset3
169458	17	411894	7	NULL	NULL	0	NULL	reliability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this article is to review the literature on the reliability and validity of scores for Waddell 's nonorganic signs , descriptions of pain behavior and symptom magnification , coefficients of variation , correlations between musculoskeletal evaluation and function , grip measurements , and the relationship between heart rate and pain intensity .
	manualset3
169459	18	411894	7	NULL	NULL	0	NULL	validity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this article is to review the literature on the reliability and validity of scores for Waddell 's nonorganic signs , descriptions of pain behavior and symptom magnification , coefficients of variation , correlations between musculoskeletal evaluation and function , grip measurements , and the relationship between heart rate and pain intensity .
	manualset3
161437	1	411895	7	NULL	NULL	0	NULL	purpose	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this case report was to demonstrate a conservative approach in the treatment of an extensive keratocystic odontogenic tumor , located in the mandible 's posterior region , using decompression and enucleation .
	manualset3
161438	2	411895	7	NULL	NULL	NULL	NULL	case report	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose of this case report was to demonstrate a conservative approach in the treatment of an extensive keratocystic odontogenic tumor , located in the mandible 's posterior region , using decompression and enucleation .
	manualset3
161439	3	411895	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this case report was to demonstrate a conservative approach in the treatment of an extensive keratocystic odontogenic tumor , located in the mandible 's posterior region , using decompression and enucleation .
	manualset3
161440	4	411895	7	NULL	NULL	0	NULL	extensive keratocystic odontogenic tumor	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this case report was to demonstrate a conservative approach in the treatment of an extensive keratocystic odontogenic tumor , located in the mandible 's posterior region , using decompression and enucleation .
	manualset3
161441	5	411895	7	NULL	NULL	0	NULL	mandible 's posterior region 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this case report was to demonstrate a conservative approach in the treatment of an extensive keratocystic odontogenic tumor , located in the mandible 's posterior region , using decompression and enucleation .
	manualset3
161442	6	411895	7	NULL	NULL	0	NULL	decompression	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this case report was to demonstrate a conservative approach in the treatment of an extensive keratocystic odontogenic tumor , located in the mandible 's posterior region , using decompression and enucleation .
	manualset3
161443	7	411895	7	NULL	NULL	0	NULL	enucleation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this case report was to demonstrate a conservative approach in the treatment of an extensive keratocystic odontogenic tumor , located in the mandible 's posterior region , using decompression and enucleation .
	manualset3
161444	8	411895	7	NULL	NULL	NULL	NULL	conservative approach	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose of this case report was to demonstrate a conservative approach in the treatment of an extensive keratocystic odontogenic tumor , located in the mandible 's posterior region , using decompression and enucleation .
	manualset3
161445	1	411896	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this investigation was to assess the sensitivity and specificity of myoglobin antiserum as a marker of rhabdomyosarcomas .
	manualset3
161446	2	411896	7	NULL	NULL	0	NULL	investigation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this investigation was to assess the sensitivity and specificity of myoglobin antiserum as a marker of rhabdomyosarcomas .
	manualset3
161447	3	411896	7	NULL	NULL	0	NULL	sensitivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this investigation was to assess the sensitivity and specificity of myoglobin antiserum as a marker of rhabdomyosarcomas .
	manualset3
161448	4	411896	7	NULL	NULL	0	NULL	specificity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this investigation was to assess the sensitivity and specificity of myoglobin antiserum as a marker of rhabdomyosarcomas .
	manualset3
161449	5	411896	7	NULL	NULL	0	NULL	myoglobin antiserum	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this investigation was to assess the sensitivity and specificity of myoglobin antiserum as a marker of rhabdomyosarcomas .
	manualset3
161450	6	411896	7	NULL	NULL	0	NULL	marker	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this investigation was to assess the sensitivity and specificity of myoglobin antiserum as a marker of rhabdomyosarcomas .
	manualset3
161451	7	411896	7	NULL	NULL	0	NULL	rhabdomyosarcomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this investigation was to assess the sensitivity and specificity of myoglobin antiserum as a marker of rhabdomyosarcomas .
	manualset3
161452	1	411897	7	NULL	NULL	0	NULL	purpose 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this investigation was to study effects of acetaminophen consumption on ratings of perceived exertion and estimated time limit responses at the lactate threshold .
	manualset3
161453	2	411897	7	NULL	NULL	0	NULL	investigation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this investigation was to study effects of acetaminophen consumption on ratings of perceived exertion and estimated time limit responses at the lactate threshold .
	manualset3
161454	3	411897	7	NULL	NULL	0	NULL	acetaminophen consumption	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this investigation was to study effects of acetaminophen consumption on ratings of perceived exertion and estimated time limit responses at the lactate threshold .
	manualset3
161455	4	411897	7	NULL	NULL	NULL	NULL	perceived exertion	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose of this investigation was to study effects of acetaminophen consumption on ratings of perceived exertion and estimated time limit responses at the lactate threshold .
	manualset3
161456	5	411897	7	NULL	NULL	0	NULL	time limit responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this investigation was to study effects of acetaminophen consumption on ratings of perceived exertion and estimated time limit responses at the lactate threshold .
	manualset3
161457	6	411897	7	NULL	NULL	0	NULL	 lactate threshold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this investigation was to study effects of acetaminophen consumption on ratings of perceived exertion and estimated time limit responses at the lactate threshold .
	manualset3
161458	1	411898	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this investigation was to study the control of cross-sectional dimensions and edge bevel by various manufacturers in the production of chrome-cobalt archwires and this effect on transmitting torque through an .018 inc slot bracket system .
	manualset3
161459	2	411898	7	NULL	NULL	0	NULL	 investigation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this investigation was to study the control of cross-sectional dimensions and edge bevel by various manufacturers in the production of chrome-cobalt archwires and this effect on transmitting torque through an .018 inc slot bracket system .
	manualset3
161460	3	411898	7	NULL	NULL	0	NULL	control 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this investigation was to study the control of cross-sectional dimensions and edge bevel by various manufacturers in the production of chrome-cobalt archwires and this effect on transmitting torque through an .018 inc slot bracket system .
	manualset3
161461	4	411898	7	NULL	NULL	0	NULL	cross-sectional dimensions	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this investigation was to study the control of cross-sectional dimensions and edge bevel by various manufacturers in the production of chrome-cobalt archwires and this effect on transmitting torque through an .018 inc slot bracket system .
	manualset3
161462	5	411898	7	NULL	NULL	0	NULL	edge bevel 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this investigation was to study the control of cross-sectional dimensions and edge bevel by various manufacturers in the production of chrome-cobalt archwires and this effect on transmitting torque through an .018 inc slot bracket system .
	manualset3
161463	6	411898	7	NULL	NULL	0	NULL	 manufacturers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this investigation was to study the control of cross-sectional dimensions and edge bevel by various manufacturers in the production of chrome-cobalt archwires and this effect on transmitting torque through an .018 inc slot bracket system .
	manualset3
161464	7	411898	7	NULL	NULL	0	NULL	production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this investigation was to study the control of cross-sectional dimensions and edge bevel by various manufacturers in the production of chrome-cobalt archwires and this effect on transmitting torque through an .018 inc slot bracket system .
	manualset3
161465	8	411898	7	NULL	NULL	0	NULL	chrome-cobalt archwires	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this investigation was to study the control of cross-sectional dimensions and edge bevel by various manufacturers in the production of chrome-cobalt archwires and this effect on transmitting torque through an .018 inc slot bracket system .
	manualset3
161466	9	411898	7	NULL	NULL	0	NULL	torque	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this investigation was to study the control of cross-sectional dimensions and edge bevel by various manufacturers in the production of chrome-cobalt archwires and this effect on transmitting torque through an .018 inc slot bracket system .
	manualset3
161467	10	411898	7	NULL	NULL	0	NULL	.018 inc	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this investigation was to study the control of cross-sectional dimensions and edge bevel by various manufacturers in the production of chrome-cobalt archwires and this effect on transmitting torque through an .018 inc slot bracket system .
	manualset3
161468	11	411898	7	NULL	NULL	0	NULL	slot bracket system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this investigation was to study the control of cross-sectional dimensions and edge bevel by various manufacturers in the production of chrome-cobalt archwires and this effect on transmitting torque through an .018 inc slot bracket system .
	manualset3
161469	1	411899	7	NULL	NULL	0	NULL	 purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this paper is to provide diagnostic guidelines and examination protocols for differential diagnosis of cutaneous facial sinus tracts of dental origin .
	manualset3
161470	2	411899	7	NULL	NULL	0	NULL	paper 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this paper is to provide diagnostic guidelines and examination protocols for differential diagnosis of cutaneous facial sinus tracts of dental origin .
	manualset3
161471	3	411899	7	NULL	NULL	NULL	NULL	diagnostic guidelines	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose of this paper is to provide diagnostic guidelines and examination protocols for differential diagnosis of cutaneous facial sinus tracts of dental origin .
	manualset3
161472	4	411899	7	NULL	NULL	NULL	NULL	examination protocols	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose of this paper is to provide diagnostic guidelines and examination protocols for differential diagnosis of cutaneous facial sinus tracts of dental origin .
	manualset3
161473	5	411899	7	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this paper is to provide diagnostic guidelines and examination protocols for differential diagnosis of cutaneous facial sinus tracts of dental origin .
	manualset3
161474	6	411899	7	NULL	NULL	0	NULL	cutaneous facial sinus tracts of dental origin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this paper is to provide diagnostic guidelines and examination protocols for differential diagnosis of cutaneous facial sinus tracts of dental origin .
	manualset3
161475	1	411900	7	NULL	NULL	0	NULL	 purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this research was to investigate the congruent/incongruent perceptions of hearing-loss related quality of life between members of couples and to determine how incongruence was affected by individual psychosocial characteristics , specifically measures of mood ( negative affect and positive affect ) , stress , and communication in the marriage .
	manualset3
161476	2	411900	7	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this research was to investigate the congruent/incongruent perceptions of hearing-loss related quality of life between members of couples and to determine how incongruence was affected by individual psychosocial characteristics , specifically measures of mood ( negative affect and positive affect ) , stress , and communication in the marriage .
	manualset3
161477	3	411900	7	NULL	NULL	0	NULL	congruent/incongruent perceptions	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this research was to investigate the congruent/incongruent perceptions of hearing-loss related quality of life between members of couples and to determine how incongruence was affected by individual psychosocial characteristics , specifically measures of mood ( negative affect and positive affect ) , stress , and communication in the marriage .
	manualset3
161478	4	411900	7	NULL	NULL	0	NULL	hearing-loss related quality of life 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this research was to investigate the congruent/incongruent perceptions of hearing-loss related quality of life between members of couples and to determine how incongruence was affected by individual psychosocial characteristics , specifically measures of mood ( negative affect and positive affect ) , stress , and communication in the marriage .
	manualset3
161479	5	411900	7	NULL	NULL	0	NULL	members of couples	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this research was to investigate the congruent/incongruent perceptions of hearing-loss related quality of life between members of couples and to determine how incongruence was affected by individual psychosocial characteristics , specifically measures of mood ( negative affect and positive affect ) , stress , and communication in the marriage .
	manualset3
161481	7	411900	7	NULL	NULL	NULL	NULL	individual psychosocial characteristics	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose of this research was to investigate the congruent/incongruent perceptions of hearing-loss related quality of life between members of couples and to determine how incongruence was affected by individual psychosocial characteristics , specifically measures of mood ( negative affect and positive affect ) , stress , and communication in the marriage .
	manualset3
161482	8	411900	7	NULL	NULL	0	NULL	measures of mood 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this research was to investigate the congruent/incongruent perceptions of hearing-loss related quality of life between members of couples and to determine how incongruence was affected by individual psychosocial characteristics , specifically measures of mood ( negative affect and positive affect ) , stress , and communication in the marriage .
	manualset3
161483	9	411900	7	NULL	NULL	0	NULL	negative affect	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this research was to investigate the congruent/incongruent perceptions of hearing-loss related quality of life between members of couples and to determine how incongruence was affected by individual psychosocial characteristics , specifically measures of mood ( negative affect and positive affect ) , stress , and communication in the marriage .
	manualset3
161484	10	411900	7	NULL	NULL	0	NULL	positive affect	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this research was to investigate the congruent/incongruent perceptions of hearing-loss related quality of life between members of couples and to determine how incongruence was affected by individual psychosocial characteristics , specifically measures of mood ( negative affect and positive affect ) , stress , and communication in the marriage .
	manualset3
161485	11	411900	7	NULL	NULL	0	NULL	 stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this research was to investigate the congruent/incongruent perceptions of hearing-loss related quality of life between members of couples and to determine how incongruence was affected by individual psychosocial characteristics , specifically measures of mood ( negative affect and positive affect ) , stress , and communication in the marriage .
	manualset3
161486	12	411900	7	NULL	NULL	0	NULL	communication	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this research was to investigate the congruent/incongruent perceptions of hearing-loss related quality of life between members of couples and to determine how incongruence was affected by individual psychosocial characteristics , specifically measures of mood ( negative affect and positive affect ) , stress , and communication in the marriage .
	manualset3
161487	13	411900	7	NULL	NULL	0	NULL	marriage	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this research was to investigate the congruent/incongruent perceptions of hearing-loss related quality of life between members of couples and to determine how incongruence was affected by individual psychosocial characteristics , specifically measures of mood ( negative affect and positive affect ) , stress , and communication in the marriage .
	manualset3
169460	14	411900	7	NULL	NULL	0	NULL	incongruence 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this research was to investigate the congruent/incongruent perceptions of hearing-loss related quality of life between members of couples and to determine how incongruence was affected by individual psychosocial characteristics , specifically measures of mood ( negative affect and positive affect ) , stress , and communication in the marriage .
	manualset3
161488	1	411901	7	NULL	NULL	0	NULL	purpose	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this review is to examine current research about the potential use of thalidomide as an anti-angiogenic agent , including potential role in treating mustard gas eye injury .
	manualset3
161489	2	411901	7	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this review is to examine current research about the potential use of thalidomide as an anti-angiogenic agent , including potential role in treating mustard gas eye injury .
	manualset3
161490	3	411901	7	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this review is to examine current research about the potential use of thalidomide as an anti-angiogenic agent , including potential role in treating mustard gas eye injury .
	manualset3
161491	4	411901	7	NULL	NULL	0	NULL	thalidomide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this review is to examine current research about the potential use of thalidomide as an anti-angiogenic agent , including potential role in treating mustard gas eye injury .
	manualset3
161492	5	411901	7	NULL	NULL	0	NULL	anti-angiogenic agent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this review is to examine current research about the potential use of thalidomide as an anti-angiogenic agent , including potential role in treating mustard gas eye injury .
	manualset3
161493	6	411901	7	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this review is to examine current research about the potential use of thalidomide as an anti-angiogenic agent , including potential role in treating mustard gas eye injury .
	manualset3
161494	7	411901	7	NULL	NULL	0	NULL	mustard gas eye injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this review is to examine current research about the potential use of thalidomide as an anti-angiogenic agent , including potential role in treating mustard gas eye injury .
	manualset3
161495	1	411902	7	NULL	NULL	NULL	NULL	purpose	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose of this review is to provide current information on fecal incontinence and its management in the elderly .
	manualset3
161496	2	411902	7	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this review is to provide current information on fecal incontinence and its management in the elderly .
	manualset3
161497	3	411902	7	NULL	NULL	0	NULL	information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this review is to provide current information on fecal incontinence and its management in the elderly .
	manualset3
161498	4	411902	7	NULL	NULL	0	NULL	 fecal incontinence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this review is to provide current information on fecal incontinence and its management in the elderly .
	manualset3
161499	5	411902	7	NULL	NULL	0	NULL	management	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this review is to provide current information on fecal incontinence and its management in the elderly .
	manualset3
161500	1	411903	7	NULL	NULL	0	NULL	Abdominal distention	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Abdominal distention was the only symptom or sign found to be associated with mortality .
	manualset3
161501	2	411903	7	NULL	NULL	0	NULL	symptom	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Abdominal distention was the only symptom or sign found to be associated with mortality .
	manualset3
161502	3	411903	7	NULL	NULL	0	NULL	sign	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Abdominal distention was the only symptom or sign found to be associated with mortality .
	manualset3
161503	4	411903	7	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Abdominal distention was the only symptom or sign found to be associated with mortality .
	manualset3
161504	1	411904	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study is to identify novel genetic loci associated with the sight threatening complications of diabetic retinopathy .
	manualset3
161505	2	411904	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study is to identify novel genetic loci associated with the sight threatening complications of diabetic retinopathy .
	manualset3
161506	3	411904	7	NULL	NULL	0	NULL	novel genetic loci 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study is to identify novel genetic loci associated with the sight threatening complications of diabetic retinopathy .
	manualset3
161507	4	411904	7	NULL	NULL	0	NULL	sight threatening complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study is to identify novel genetic loci associated with the sight threatening complications of diabetic retinopathy .
	manualset3
161508	5	411904	7	NULL	NULL	NULL	NULL	diabetic retinopathy	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose of this study is to identify novel genetic loci associated with the sight threatening complications of diabetic retinopathy .
	manualset3
161509	1	411905	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study is to investigate the apoptotic effect induced by the interactions of arsenic and UVB on cultured human keratinocytes .
	manualset3
161510	2	411905	7	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study is to investigate the apoptotic effect induced by the interactions of arsenic and UVB on cultured human keratinocytes .
	manualset3
161511	3	411905	7	NULL	NULL	0	NULL	apoptotic effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study is to investigate the apoptotic effect induced by the interactions of arsenic and UVB on cultured human keratinocytes .
	manualset3
161512	4	411905	7	NULL	NULL	0	NULL	interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study is to investigate the apoptotic effect induced by the interactions of arsenic and UVB on cultured human keratinocytes .
	manualset3
161513	5	411905	7	NULL	NULL	0	NULL	arsenic	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study is to investigate the apoptotic effect induced by the interactions of arsenic and UVB on cultured human keratinocytes .
	manualset3
161514	6	411905	7	NULL	NULL	0	NULL	UVB	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study is to investigate the apoptotic effect induced by the interactions of arsenic and UVB on cultured human keratinocytes .
	manualset3
161515	7	411905	7	NULL	NULL	0	NULL	cultured human keratinocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study is to investigate the apoptotic effect induced by the interactions of arsenic and UVB on cultured human keratinocytes .
	manualset3
161516	1	411906	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was : 1 ) to determine whether anaerobic glycolysis contributes to the tolerance to anoxia and preservation of cellular ATP in immature tubules and 2 ) to evaluate whether the tolerance demonstrated by immature tubules is dependent on preservation of cellular ATP .
	manualset3
161517	2	411906	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was : 1 ) to determine whether anaerobic glycolysis contributes to the tolerance to anoxia and preservation of cellular ATP in immature tubules and 2 ) to evaluate whether the tolerance demonstrated by immature tubules is dependent on preservation of cellular ATP .
	manualset3
161518	3	411906	7	NULL	NULL	NULL	NULL	anaerobic glycolysis	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose of this study was : 1 ) to determine whether anaerobic glycolysis contributes to the tolerance to anoxia and preservation of cellular ATP in immature tubules and 2 ) to evaluate whether the tolerance demonstrated by immature tubules is dependent on preservation of cellular ATP .
	manualset3
161519	4	411906	7	NULL	NULL	NULL	NULL	 tolerance	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose of this study was : 1 ) to determine whether anaerobic glycolysis contributes to the tolerance to anoxia and preservation of cellular ATP in immature tubules and 2 ) to evaluate whether the tolerance demonstrated by immature tubules is dependent on preservation of cellular ATP .
	manualset3
161520	5	411906	7	NULL	NULL	0	NULL	anoxia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was : 1 ) to determine whether anaerobic glycolysis contributes to the tolerance to anoxia and preservation of cellular ATP in immature tubules and 2 ) to evaluate whether the tolerance demonstrated by immature tubules is dependent on preservation of cellular ATP .
	manualset3
161521	6	411906	7	NULL	NULL	0	NULL	 preservation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was : 1 ) to determine whether anaerobic glycolysis contributes to the tolerance to anoxia and preservation of cellular ATP in immature tubules and 2 ) to evaluate whether the tolerance demonstrated by immature tubules is dependent on preservation of cellular ATP .
	manualset3
161522	7	411906	7	NULL	NULL	0	NULL	cellular ATP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was : 1 ) to determine whether anaerobic glycolysis contributes to the tolerance to anoxia and preservation of cellular ATP in immature tubules and 2 ) to evaluate whether the tolerance demonstrated by immature tubules is dependent on preservation of cellular ATP .
	manualset3
161523	8	411906	7	NULL	NULL	0	NULL	immature tubules	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was : 1 ) to determine whether anaerobic glycolysis contributes to the tolerance to anoxia and preservation of cellular ATP in immature tubules and 2 ) to evaluate whether the tolerance demonstrated by immature tubules is dependent on preservation of cellular ATP .
	manualset3
161524	9	411906	7	NULL	NULL	NULL	NULL	 tolerance	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose of this study was : 1 ) to determine whether anaerobic glycolysis contributes to the tolerance to anoxia and preservation of cellular ATP in immature tubules and 2 ) to evaluate whether the tolerance demonstrated by immature tubules is dependent on preservation of cellular ATP .
	manualset3
161525	10	411906	7	NULL	NULL	0	NULL	 immature tubules	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was : 1 ) to determine whether anaerobic glycolysis contributes to the tolerance to anoxia and preservation of cellular ATP in immature tubules and 2 ) to evaluate whether the tolerance demonstrated by immature tubules is dependent on preservation of cellular ATP .
	manualset3
161526	11	411906	7	NULL	NULL	0	NULL	preservation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was : 1 ) to determine whether anaerobic glycolysis contributes to the tolerance to anoxia and preservation of cellular ATP in immature tubules and 2 ) to evaluate whether the tolerance demonstrated by immature tubules is dependent on preservation of cellular ATP .
	manualset3
161527	12	411906	7	NULL	NULL	0	NULL	cellular ATP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was : 1 ) to determine whether anaerobic glycolysis contributes to the tolerance to anoxia and preservation of cellular ATP in immature tubules and 2 ) to evaluate whether the tolerance demonstrated by immature tubules is dependent on preservation of cellular ATP .
	manualset3
161528	1	411907	7	NULL	NULL	0	NULL	 purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to analyze the involvement of specific PKC isoenzymes and their effector protein CPI-17 in thrombin-induced MLC phosphorylation and actin stress fiber assembly in RPE cells .
	manualset3
161529	2	411907	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to analyze the involvement of specific PKC isoenzymes and their effector protein CPI-17 in thrombin-induced MLC phosphorylation and actin stress fiber assembly in RPE cells .
	manualset3
161530	3	411907	7	NULL	NULL	0	NULL	involvement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to analyze the involvement of specific PKC isoenzymes and their effector protein CPI-17 in thrombin-induced MLC phosphorylation and actin stress fiber assembly in RPE cells .
	manualset3
161531	4	411907	7	NULL	NULL	0	NULL	PKC isoenzymes	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to analyze the involvement of specific PKC isoenzymes and their effector protein CPI-17 in thrombin-induced MLC phosphorylation and actin stress fiber assembly in RPE cells .
	manualset3
161532	5	411907	7	NULL	NULL	0	NULL	effector protein CPI-17	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to analyze the involvement of specific PKC isoenzymes and their effector protein CPI-17 in thrombin-induced MLC phosphorylation and actin stress fiber assembly in RPE cells .
	manualset3
161533	6	411907	7	NULL	NULL	0	NULL	thrombin-induced MLC phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to analyze the involvement of specific PKC isoenzymes and their effector protein CPI-17 in thrombin-induced MLC phosphorylation and actin stress fiber assembly in RPE cells .
	manualset3
161534	7	411907	7	NULL	NULL	0	NULL	actin stress fiber assembly	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to analyze the involvement of specific PKC isoenzymes and their effector protein CPI-17 in thrombin-induced MLC phosphorylation and actin stress fiber assembly in RPE cells .
	manualset3
161535	8	411907	7	NULL	NULL	0	NULL	RPE cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to analyze the involvement of specific PKC isoenzymes and their effector protein CPI-17 in thrombin-induced MLC phosphorylation and actin stress fiber assembly in RPE cells .
	manualset3
161536	1	411908	7	NULL	NULL	0	NULL	purpose 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to assess the presence and location of impaired myocardial sympathetic innervation by using 123I metaiodobenzylguanidine ( 123I MIBG ) in 15 patients with coronary vasospasm induced by intracoronary acetylcholine .
	manualset3
161537	2	411908	7	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to assess the presence and location of impaired myocardial sympathetic innervation by using 123I metaiodobenzylguanidine ( 123I MIBG ) in 15 patients with coronary vasospasm induced by intracoronary acetylcholine .
	manualset3
161538	3	411908	7	NULL	NULL	0	NULL	presence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to assess the presence and location of impaired myocardial sympathetic innervation by using 123I metaiodobenzylguanidine ( 123I MIBG ) in 15 patients with coronary vasospasm induced by intracoronary acetylcholine .
	manualset3
161539	4	411908	7	NULL	NULL	0	NULL	 location	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to assess the presence and location of impaired myocardial sympathetic innervation by using 123I metaiodobenzylguanidine ( 123I MIBG ) in 15 patients with coronary vasospasm induced by intracoronary acetylcholine .
	manualset3
161540	5	411908	7	NULL	NULL	0	NULL	impaired myocardial sympathetic innervation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to assess the presence and location of impaired myocardial sympathetic innervation by using 123I metaiodobenzylguanidine ( 123I MIBG ) in 15 patients with coronary vasospasm induced by intracoronary acetylcholine .
	manualset3
161541	6	411908	7	NULL	NULL	0	NULL	123I metaiodobenzylguanidine ( 123I MIBG )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to assess the presence and location of impaired myocardial sympathetic innervation by using 123I metaiodobenzylguanidine ( 123I MIBG ) in 15 patients with coronary vasospasm induced by intracoronary acetylcholine .
	manualset3
161542	7	411908	7	NULL	NULL	0	NULL	15 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to assess the presence and location of impaired myocardial sympathetic innervation by using 123I metaiodobenzylguanidine ( 123I MIBG ) in 15 patients with coronary vasospasm induced by intracoronary acetylcholine .
	manualset3
161543	8	411908	7	NULL	NULL	0	NULL	coronary vasospasm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to assess the presence and location of impaired myocardial sympathetic innervation by using 123I metaiodobenzylguanidine ( 123I MIBG ) in 15 patients with coronary vasospasm induced by intracoronary acetylcholine .
	manualset3
161544	9	411908	7	NULL	NULL	0	NULL	intracoronary acetylcholine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to assess the presence and location of impaired myocardial sympathetic innervation by using 123I metaiodobenzylguanidine ( 123I MIBG ) in 15 patients with coronary vasospasm induced by intracoronary acetylcholine .
	manualset3
161545	1	411909	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to assess whether gastric reactance is a reliable , clinically relevant predictor of complications and a potentially useful tool to assess hypoperfusion in cardiovascular surgery patients .
	manualset3
161546	2	411909	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to assess whether gastric reactance is a reliable , clinically relevant predictor of complications and a potentially useful tool to assess hypoperfusion in cardiovascular surgery patients .
	manualset3
161547	3	411909	7	NULL	NULL	0	NULL	gastric reactance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to assess whether gastric reactance is a reliable , clinically relevant predictor of complications and a potentially useful tool to assess hypoperfusion in cardiovascular surgery patients .
	manualset3
161548	4	411909	7	NULL	NULL	0	NULL	predictor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to assess whether gastric reactance is a reliable , clinically relevant predictor of complications and a potentially useful tool to assess hypoperfusion in cardiovascular surgery patients .
	manualset3
161549	5	411909	7	NULL	NULL	0	NULL	complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to assess whether gastric reactance is a reliable , clinically relevant predictor of complications and a potentially useful tool to assess hypoperfusion in cardiovascular surgery patients .
	manualset3
161550	6	411909	7	NULL	NULL	0	NULL	 tool 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to assess whether gastric reactance is a reliable , clinically relevant predictor of complications and a potentially useful tool to assess hypoperfusion in cardiovascular surgery patients .
	manualset3
161551	7	411909	7	NULL	NULL	0	NULL	hypoperfusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to assess whether gastric reactance is a reliable , clinically relevant predictor of complications and a potentially useful tool to assess hypoperfusion in cardiovascular surgery patients .
	manualset3
161552	8	411909	7	NULL	NULL	0	NULL	cardiovascular surgery patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to assess whether gastric reactance is a reliable , clinically relevant predictor of complications and a potentially useful tool to assess hypoperfusion in cardiovascular surgery patients .
	manualset3
161553	1	411910	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to demonstrate that SPIO agent ferumoxides-protamine sulfate ( FePro ) incorporation into macrophages does not alter immunological properties of these cells with regard to differentiation , chemotaxis , and ability to respond to the activation stimuli and to modulate T cell response .
	manualset3
161554	2	411910	7	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to demonstrate that SPIO agent ferumoxides-protamine sulfate ( FePro ) incorporation into macrophages does not alter immunological properties of these cells with regard to differentiation , chemotaxis , and ability to respond to the activation stimuli and to modulate T cell response .
	manualset3
161555	3	411910	7	NULL	NULL	0	NULL	SPIO agent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to demonstrate that SPIO agent ferumoxides-protamine sulfate ( FePro ) incorporation into macrophages does not alter immunological properties of these cells with regard to differentiation , chemotaxis , and ability to respond to the activation stimuli and to modulate T cell response .
	manualset3
161556	4	411910	7	NULL	NULL	0	NULL	ferumoxides-protamine sulfate ( FePro )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to demonstrate that SPIO agent ferumoxides-protamine sulfate ( FePro ) incorporation into macrophages does not alter immunological properties of these cells with regard to differentiation , chemotaxis , and ability to respond to the activation stimuli and to modulate T cell response .
	manualset3
161557	5	411910	7	NULL	NULL	0	NULL	incorporation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to demonstrate that SPIO agent ferumoxides-protamine sulfate ( FePro ) incorporation into macrophages does not alter immunological properties of these cells with regard to differentiation , chemotaxis , and ability to respond to the activation stimuli and to modulate T cell response .
	manualset3
161558	6	411910	7	NULL	NULL	0	NULL	macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to demonstrate that SPIO agent ferumoxides-protamine sulfate ( FePro ) incorporation into macrophages does not alter immunological properties of these cells with regard to differentiation , chemotaxis , and ability to respond to the activation stimuli and to modulate T cell response .
	manualset3
161559	7	411910	7	NULL	NULL	0	NULL	immunological properties	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to demonstrate that SPIO agent ferumoxides-protamine sulfate ( FePro ) incorporation into macrophages does not alter immunological properties of these cells with regard to differentiation , chemotaxis , and ability to respond to the activation stimuli and to modulate T cell response .
	manualset3
161560	8	411910	7	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to demonstrate that SPIO agent ferumoxides-protamine sulfate ( FePro ) incorporation into macrophages does not alter immunological properties of these cells with regard to differentiation , chemotaxis , and ability to respond to the activation stimuli and to modulate T cell response .
	manualset3
161561	9	411910	7	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to demonstrate that SPIO agent ferumoxides-protamine sulfate ( FePro ) incorporation into macrophages does not alter immunological properties of these cells with regard to differentiation , chemotaxis , and ability to respond to the activation stimuli and to modulate T cell response .
	manualset3
161562	10	411910	7	NULL	NULL	0	NULL	chemotaxis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to demonstrate that SPIO agent ferumoxides-protamine sulfate ( FePro ) incorporation into macrophages does not alter immunological properties of these cells with regard to differentiation , chemotaxis , and ability to respond to the activation stimuli and to modulate T cell response .
	manualset3
161563	11	411910	7	NULL	NULL	0	NULL	 activation stimuli	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to demonstrate that SPIO agent ferumoxides-protamine sulfate ( FePro ) incorporation into macrophages does not alter immunological properties of these cells with regard to differentiation , chemotaxis , and ability to respond to the activation stimuli and to modulate T cell response .
	manualset3
161564	12	411910	7	NULL	NULL	0	NULL	T cell response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to demonstrate that SPIO agent ferumoxides-protamine sulfate ( FePro ) incorporation into macrophages does not alter immunological properties of these cells with regard to differentiation , chemotaxis , and ability to respond to the activation stimuli and to modulate T cell response .
	manualset3
161565	1	411911	7	NULL	NULL	0	NULL	( 3H ) Glutamic acid ( PCA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3H ) Glutamic acid ( PCA ) was followed with time after a single subcutaneous injection .
	manualset3
161566	2	411911	7	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3H ) Glutamic acid ( PCA ) was followed with time after a single subcutaneous injection .
	manualset3
161567	3	411911	7	NULL	NULL	0	NULL	single subcutaneous injection 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3H ) Glutamic acid ( PCA ) was followed with time after a single subcutaneous injection .
	manualset3
161568	1	411912	7	NULL	NULL	0	NULL	Clinical symptomatology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical symptomatology in hemorrhagic telangiectasia ) .
	manualset3
161569	2	411912	7	NULL	NULL	NULL	NULL	hemorrhagic telangiectasia 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Clinical symptomatology in hemorrhagic telangiectasia ) .
	manualset3
161570	1	411913	7	NULL	NULL	0	NULL	Abdominal insufflation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Abdominal insufflation at 5 , 10 , 15 , and 20 mm Hg caused an increase in ETCO ( 2 ) to 31.7 + / - 0.8 mm Hg , 35.6 + / - 1.2 * mm Hg , 37.5 + / - 1.5 * mm Hg , and 40.1 + / - 1.8 * mm Hg and in PaCO ( 2 ) to 41.1 + / - 1.3 * mm Hg , 44.2 + / - 1.4 * mm Hg , 49.9 + / - 1.8 * mm Hg , and 53.0 + / - 2.1 * mm Hg , respectively .
	manualset3
161571	2	411913	7	NULL	NULL	0	NULL	5 , 10 , 15 , and 20 mm Hg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Abdominal insufflation at 5 , 10 , 15 , and 20 mm Hg caused an increase in ETCO ( 2 ) to 31.7 + / - 0.8 mm Hg , 35.6 + / - 1.2 * mm Hg , 37.5 + / - 1.5 * mm Hg , and 40.1 + / - 1.8 * mm Hg and in PaCO ( 2 ) to 41.1 + / - 1.3 * mm Hg , 44.2 + / - 1.4 * mm Hg , 49.9 + / - 1.8 * mm Hg , and 53.0 + / - 2.1 * mm Hg , respectively .
	manualset3
161572	3	411913	7	NULL	NULL	0	NULL	ETCO ( 2 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Abdominal insufflation at 5 , 10 , 15 , and 20 mm Hg caused an increase in ETCO ( 2 ) to 31.7 + / - 0.8 mm Hg , 35.6 + / - 1.2 * mm Hg , 37.5 + / - 1.5 * mm Hg , and 40.1 + / - 1.8 * mm Hg and in PaCO ( 2 ) to 41.1 + / - 1.3 * mm Hg , 44.2 + / - 1.4 * mm Hg , 49.9 + / - 1.8 * mm Hg , and 53.0 + / - 2.1 * mm Hg , respectively .
	manualset3
161573	4	411913	7	NULL	NULL	0	NULL	 31.7 + / - 0.8 mm Hg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Abdominal insufflation at 5 , 10 , 15 , and 20 mm Hg caused an increase in ETCO ( 2 ) to 31.7 + / - 0.8 mm Hg , 35.6 + / - 1.2 * mm Hg , 37.5 + / - 1.5 * mm Hg , and 40.1 + / - 1.8 * mm Hg and in PaCO ( 2 ) to 41.1 + / - 1.3 * mm Hg , 44.2 + / - 1.4 * mm Hg , 49.9 + / - 1.8 * mm Hg , and 53.0 + / - 2.1 * mm Hg , respectively .
	manualset3
161574	5	411913	7	NULL	NULL	0	NULL	35.6 + / - 1.2 * mm Hg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Abdominal insufflation at 5 , 10 , 15 , and 20 mm Hg caused an increase in ETCO ( 2 ) to 31.7 + / - 0.8 mm Hg , 35.6 + / - 1.2 * mm Hg , 37.5 + / - 1.5 * mm Hg , and 40.1 + / - 1.8 * mm Hg and in PaCO ( 2 ) to 41.1 + / - 1.3 * mm Hg , 44.2 + / - 1.4 * mm Hg , 49.9 + / - 1.8 * mm Hg , and 53.0 + / - 2.1 * mm Hg , respectively .
	manualset3
161575	6	411913	7	NULL	NULL	0	NULL	37.5 + / - 1.5 * mm Hg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Abdominal insufflation at 5 , 10 , 15 , and 20 mm Hg caused an increase in ETCO ( 2 ) to 31.7 + / - 0.8 mm Hg , 35.6 + / - 1.2 * mm Hg , 37.5 + / - 1.5 * mm Hg , and 40.1 + / - 1.8 * mm Hg and in PaCO ( 2 ) to 41.1 + / - 1.3 * mm Hg , 44.2 + / - 1.4 * mm Hg , 49.9 + / - 1.8 * mm Hg , and 53.0 + / - 2.1 * mm Hg , respectively .
	manualset3
161576	7	411913	7	NULL	NULL	0	NULL	40.1 + / - 1.8 * mm Hg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Abdominal insufflation at 5 , 10 , 15 , and 20 mm Hg caused an increase in ETCO ( 2 ) to 31.7 + / - 0.8 mm Hg , 35.6 + / - 1.2 * mm Hg , 37.5 + / - 1.5 * mm Hg , and 40.1 + / - 1.8 * mm Hg and in PaCO ( 2 ) to 41.1 + / - 1.3 * mm Hg , 44.2 + / - 1.4 * mm Hg , 49.9 + / - 1.8 * mm Hg , and 53.0 + / - 2.1 * mm Hg , respectively .
	manualset3
161577	8	411913	7	NULL	NULL	0	NULL	PaCO ( 2 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Abdominal insufflation at 5 , 10 , 15 , and 20 mm Hg caused an increase in ETCO ( 2 ) to 31.7 + / - 0.8 mm Hg , 35.6 + / - 1.2 * mm Hg , 37.5 + / - 1.5 * mm Hg , and 40.1 + / - 1.8 * mm Hg and in PaCO ( 2 ) to 41.1 + / - 1.3 * mm Hg , 44.2 + / - 1.4 * mm Hg , 49.9 + / - 1.8 * mm Hg , and 53.0 + / - 2.1 * mm Hg , respectively .
	manualset3
161578	9	411913	7	NULL	NULL	0	NULL	41.1 + / - 1.3 * mm Hg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Abdominal insufflation at 5 , 10 , 15 , and 20 mm Hg caused an increase in ETCO ( 2 ) to 31.7 + / - 0.8 mm Hg , 35.6 + / - 1.2 * mm Hg , 37.5 + / - 1.5 * mm Hg , and 40.1 + / - 1.8 * mm Hg and in PaCO ( 2 ) to 41.1 + / - 1.3 * mm Hg , 44.2 + / - 1.4 * mm Hg , 49.9 + / - 1.8 * mm Hg , and 53.0 + / - 2.1 * mm Hg , respectively .
	manualset3
161579	10	411913	7	NULL	NULL	0	NULL	44.2 + / - 1.4 * mm Hg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Abdominal insufflation at 5 , 10 , 15 , and 20 mm Hg caused an increase in ETCO ( 2 ) to 31.7 + / - 0.8 mm Hg , 35.6 + / - 1.2 * mm Hg , 37.5 + / - 1.5 * mm Hg , and 40.1 + / - 1.8 * mm Hg and in PaCO ( 2 ) to 41.1 + / - 1.3 * mm Hg , 44.2 + / - 1.4 * mm Hg , 49.9 + / - 1.8 * mm Hg , and 53.0 + / - 2.1 * mm Hg , respectively .
	manualset3
161580	11	411913	7	NULL	NULL	0	NULL	49.9 + / - 1.8 * mm Hg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Abdominal insufflation at 5 , 10 , 15 , and 20 mm Hg caused an increase in ETCO ( 2 ) to 31.7 + / - 0.8 mm Hg , 35.6 + / - 1.2 * mm Hg , 37.5 + / - 1.5 * mm Hg , and 40.1 + / - 1.8 * mm Hg and in PaCO ( 2 ) to 41.1 + / - 1.3 * mm Hg , 44.2 + / - 1.4 * mm Hg , 49.9 + / - 1.8 * mm Hg , and 53.0 + / - 2.1 * mm Hg , respectively .
	manualset3
161581	12	411913	7	NULL	NULL	0	NULL	53.0 + / - 2.1 * mm Hg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Abdominal insufflation at 5 , 10 , 15 , and 20 mm Hg caused an increase in ETCO ( 2 ) to 31.7 + / - 0.8 mm Hg , 35.6 + / - 1.2 * mm Hg , 37.5 + / - 1.5 * mm Hg , and 40.1 + / - 1.8 * mm Hg and in PaCO ( 2 ) to 41.1 + / - 1.3 * mm Hg , 44.2 + / - 1.4 * mm Hg , 49.9 + / - 1.8 * mm Hg , and 53.0 + / - 2.1 * mm Hg , respectively .
	manualset3
161582	1	411914	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to demonstrate the molecular interplay of the Fshr promoter involved in the transactivation by AHR in mouse granulosa cells .
	manualset3
161583	2	411914	7	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to demonstrate the molecular interplay of the Fshr promoter involved in the transactivation by AHR in mouse granulosa cells .
	manualset3
161584	3	411914	7	NULL	NULL	0	NULL	molecular interplay	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to demonstrate the molecular interplay of the Fshr promoter involved in the transactivation by AHR in mouse granulosa cells .
	manualset3
161585	4	411914	7	NULL	NULL	0	NULL	Fshr promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to demonstrate the molecular interplay of the Fshr promoter involved in the transactivation by AHR in mouse granulosa cells .
	manualset3
161586	5	411914	7	NULL	NULL	0	NULL	 transactivation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to demonstrate the molecular interplay of the Fshr promoter involved in the transactivation by AHR in mouse granulosa cells .
	manualset3
161587	6	411914	7	NULL	NULL	0	NULL	AHR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to demonstrate the molecular interplay of the Fshr promoter involved in the transactivation by AHR in mouse granulosa cells .
	manualset3
161588	7	411914	7	NULL	NULL	0	NULL	mouse granulosa cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to demonstrate the molecular interplay of the Fshr promoter involved in the transactivation by AHR in mouse granulosa cells .
	manualset3
161589	1	411915	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to describe the circadian rhythm of abdominal skin temperature and explore factors related to the timing of circadian rhythm acrophase .
	manualset3
161590	2	411915	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to describe the circadian rhythm of abdominal skin temperature and explore factors related to the timing of circadian rhythm acrophase .
	manualset3
161591	3	411915	7	NULL	NULL	0	NULL	circadian rhythm	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to describe the circadian rhythm of abdominal skin temperature and explore factors related to the timing of circadian rhythm acrophase .
	manualset3
161592	4	411915	7	NULL	NULL	0	NULL	abdominal skin temperature	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to describe the circadian rhythm of abdominal skin temperature and explore factors related to the timing of circadian rhythm acrophase .
	manualset3
161593	5	411915	7	NULL	NULL	0	NULL	 factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to describe the circadian rhythm of abdominal skin temperature and explore factors related to the timing of circadian rhythm acrophase .
	manualset3
161594	6	411915	7	NULL	NULL	0	NULL	circadian rhythm acrophase	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to describe the circadian rhythm of abdominal skin temperature and explore factors related to the timing of circadian rhythm acrophase .
	manualset3
161595	1	411916	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine the effect of hepatic IR injury on the expression of Mrps in rat liver and kidney .
	manualset3
161596	2	411916	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine the effect of hepatic IR injury on the expression of Mrps in rat liver and kidney .
	manualset3
161597	3	411916	7	NULL	NULL	0	NULL	effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine the effect of hepatic IR injury on the expression of Mrps in rat liver and kidney .
	manualset3
161598	4	411916	7	NULL	NULL	0	NULL	hepatic IR injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine the effect of hepatic IR injury on the expression of Mrps in rat liver and kidney .
	manualset3
161599	5	411916	7	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine the effect of hepatic IR injury on the expression of Mrps in rat liver and kidney .
	manualset3
161600	6	411916	7	NULL	NULL	0	NULL	Mrps	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine the effect of hepatic IR injury on the expression of Mrps in rat liver and kidney .
	manualset3
161601	7	411916	7	NULL	NULL	0	NULL	 rat liver 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine the effect of hepatic IR injury on the expression of Mrps in rat liver and kidney .
	manualset3
161602	8	411916	7	NULL	NULL	0	NULL	 kidney	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine the effect of hepatic IR injury on the expression of Mrps in rat liver and kidney .
	manualset3
161603	1	411917	7	NULL	NULL	0	NULL	 purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether a threshold size of infraspinatus defect exists beyond which abduction torque generation decreases and superior migration of the humeral head increases .
	manualset3
161604	2	411917	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether a threshold size of infraspinatus defect exists beyond which abduction torque generation decreases and superior migration of the humeral head increases .
	manualset3
161605	3	411917	7	NULL	NULL	0	NULL	 threshold size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether a threshold size of infraspinatus defect exists beyond which abduction torque generation decreases and superior migration of the humeral head increases .
	manualset3
161606	4	411917	7	NULL	NULL	0	NULL	infraspinatus defect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether a threshold size of infraspinatus defect exists beyond which abduction torque generation decreases and superior migration of the humeral head increases .
	manualset3
161607	5	411917	7	NULL	NULL	NULL	NULL	abduction torque generation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether a threshold size of infraspinatus defect exists beyond which abduction torque generation decreases and superior migration of the humeral head increases .
	manualset3
161608	6	411917	7	NULL	NULL	0	NULL	superior migration 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether a threshold size of infraspinatus defect exists beyond which abduction torque generation decreases and superior migration of the humeral head increases .
	manualset3
161609	7	411917	7	NULL	NULL	0	NULL	humeral head	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether a threshold size of infraspinatus defect exists beyond which abduction torque generation decreases and superior migration of the humeral head increases .
	manualset3
161610	1	411918	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether foals immunized orally from 2 days of age with virulent Rhodococcus equi developed a protective pulmonary immune response and to characterise the antibody response of the immunized foals to the virulence-associated proteins ( Vaps ) of the bacterium .
	manualset3
161611	2	411918	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether foals immunized orally from 2 days of age with virulent Rhodococcus equi developed a protective pulmonary immune response and to characterise the antibody response of the immunized foals to the virulence-associated proteins ( Vaps ) of the bacterium .
	manualset3
161612	3	411918	7	NULL	NULL	0	NULL	foals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether foals immunized orally from 2 days of age with virulent Rhodococcus equi developed a protective pulmonary immune response and to characterise the antibody response of the immunized foals to the virulence-associated proteins ( Vaps ) of the bacterium .
	manualset3
161613	4	411918	7	NULL	NULL	0	NULL	 2 days of age	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether foals immunized orally from 2 days of age with virulent Rhodococcus equi developed a protective pulmonary immune response and to characterise the antibody response of the immunized foals to the virulence-associated proteins ( Vaps ) of the bacterium .
	manualset3
161614	5	411918	7	NULL	NULL	0	NULL	virulent Rhodococcus equi 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether foals immunized orally from 2 days of age with virulent Rhodococcus equi developed a protective pulmonary immune response and to characterise the antibody response of the immunized foals to the virulence-associated proteins ( Vaps ) of the bacterium .
	manualset3
161615	6	411918	7	NULL	NULL	0	NULL	protective pulmonary immune response 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether foals immunized orally from 2 days of age with virulent Rhodococcus equi developed a protective pulmonary immune response and to characterise the antibody response of the immunized foals to the virulence-associated proteins ( Vaps ) of the bacterium .
	manualset3
161616	7	411918	7	NULL	NULL	0	NULL	 antibody response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether foals immunized orally from 2 days of age with virulent Rhodococcus equi developed a protective pulmonary immune response and to characterise the antibody response of the immunized foals to the virulence-associated proteins ( Vaps ) of the bacterium .
	manualset3
161617	8	411918	7	NULL	NULL	0	NULL	immunized foals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether foals immunized orally from 2 days of age with virulent Rhodococcus equi developed a protective pulmonary immune response and to characterise the antibody response of the immunized foals to the virulence-associated proteins ( Vaps ) of the bacterium .
	manualset3
161618	9	411918	7	NULL	NULL	0	NULL	virulence-associated proteins ( Vaps )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether foals immunized orally from 2 days of age with virulent Rhodococcus equi developed a protective pulmonary immune response and to characterise the antibody response of the immunized foals to the virulence-associated proteins ( Vaps ) of the bacterium .
	manualset3
161619	10	411918	7	NULL	NULL	0	NULL	bacterium	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether foals immunized orally from 2 days of age with virulent Rhodococcus equi developed a protective pulmonary immune response and to characterise the antibody response of the immunized foals to the virulence-associated proteins ( Vaps ) of the bacterium .
	manualset3
161620	1	411919	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether inactive asthmatic patients could perform high-intensity physical training equally well on land as in water , and to compare the effects of these training forms .
	manualset3
161621	2	411919	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether inactive asthmatic patients could perform high-intensity physical training equally well on land as in water , and to compare the effects of these training forms .
	manualset3
161622	3	411919	7	NULL	NULL	0	NULL	inactive asthmatic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether inactive asthmatic patients could perform high-intensity physical training equally well on land as in water , and to compare the effects of these training forms .
	manualset3
161623	4	411919	7	NULL	NULL	0	NULL	high-intensity physical training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether inactive asthmatic patients could perform high-intensity physical training equally well on land as in water , and to compare the effects of these training forms .
	manualset3
161624	5	411919	7	NULL	NULL	0	NULL	land	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether inactive asthmatic patients could perform high-intensity physical training equally well on land as in water , and to compare the effects of these training forms .
	manualset3
161625	6	411919	7	NULL	NULL	0	NULL	 water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether inactive asthmatic patients could perform high-intensity physical training equally well on land as in water , and to compare the effects of these training forms .
	manualset3
161626	7	411919	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether inactive asthmatic patients could perform high-intensity physical training equally well on land as in water , and to compare the effects of these training forms .
	manualset3
161627	8	411919	7	NULL	NULL	0	NULL	training forms	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether inactive asthmatic patients could perform high-intensity physical training equally well on land as in water , and to compare the effects of these training forms .
	manualset3
161628	1	411920	7	NULL	NULL	0	NULL	 purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether orthodontic instruments and bands contaminated with blood or saliva and bacterial spores can be heat sterilized while contained in OMS-ASAPsys instrument and band cassettes .
	manualset3
161629	2	411920	7	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether orthodontic instruments and bands contaminated with blood or saliva and bacterial spores can be heat sterilized while contained in OMS-ASAPsys instrument and band cassettes .
	manualset3
161630	3	411920	7	NULL	NULL	0	NULL	orthodontic instruments	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether orthodontic instruments and bands contaminated with blood or saliva and bacterial spores can be heat sterilized while contained in OMS-ASAPsys instrument and band cassettes .
	manualset3
161631	4	411920	7	NULL	NULL	0	NULL	bands	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether orthodontic instruments and bands contaminated with blood or saliva and bacterial spores can be heat sterilized while contained in OMS-ASAPsys instrument and band cassettes .
	manualset3
161632	5	411920	7	NULL	NULL	0	NULL	blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether orthodontic instruments and bands contaminated with blood or saliva and bacterial spores can be heat sterilized while contained in OMS-ASAPsys instrument and band cassettes .
	manualset3
161633	6	411920	7	NULL	NULL	0	NULL	saliva 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether orthodontic instruments and bands contaminated with blood or saliva and bacterial spores can be heat sterilized while contained in OMS-ASAPsys instrument and band cassettes .
	manualset3
161634	7	411920	7	NULL	NULL	0	NULL	bacterial spores	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether orthodontic instruments and bands contaminated with blood or saliva and bacterial spores can be heat sterilized while contained in OMS-ASAPsys instrument and band cassettes .
	manualset3
161635	8	411920	7	NULL	NULL	0	NULL	OMS-ASAPsys instrument 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether orthodontic instruments and bands contaminated with blood or saliva and bacterial spores can be heat sterilized while contained in OMS-ASAPsys instrument and band cassettes .
	manualset3
161636	9	411920	7	NULL	NULL	0	NULL	band cassettes	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether orthodontic instruments and bands contaminated with blood or saliva and bacterial spores can be heat sterilized while contained in OMS-ASAPsys instrument and band cassettes .
	manualset3
161637	1	411921	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether the addition of supracarinal and subcarinal low-flow oxygen insufflation to conventional intermittent positive-pressure ventilation ( IPPV ) of critically ill and anesthetized patients results in increased ventilation and improved oxygenation .
	manualset3
161638	2	411921	7	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether the addition of supracarinal and subcarinal low-flow oxygen insufflation to conventional intermittent positive-pressure ventilation ( IPPV ) of critically ill and anesthetized patients results in increased ventilation and improved oxygenation .
	manualset3
161639	3	411921	7	NULL	NULL	0	NULL	supracarinal low-flow oxygen insufflation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether the addition of supracarinal and subcarinal low-flow oxygen insufflation to conventional intermittent positive-pressure ventilation ( IPPV ) of critically ill and anesthetized patients results in increased ventilation and improved oxygenation .
	manualset3
161640	4	411921	7	NULL	NULL	0	NULL	subcarinal low-flow oxygen insufflation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether the addition of supracarinal and subcarinal low-flow oxygen insufflation to conventional intermittent positive-pressure ventilation ( IPPV ) of critically ill and anesthetized patients results in increased ventilation and improved oxygenation .
	manualset3
161641	5	411921	7	NULL	NULL	0	NULL	 intermittent positive-pressure ventilation ( IPPV ) 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether the addition of supracarinal and subcarinal low-flow oxygen insufflation to conventional intermittent positive-pressure ventilation ( IPPV ) of critically ill and anesthetized patients results in increased ventilation and improved oxygenation .
	manualset3
161642	6	411921	7	NULL	NULL	0	NULL	critically ill patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether the addition of supracarinal and subcarinal low-flow oxygen insufflation to conventional intermittent positive-pressure ventilation ( IPPV ) of critically ill and anesthetized patients results in increased ventilation and improved oxygenation .
	manualset3
161643	7	411921	7	NULL	NULL	0	NULL	anesthetized patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether the addition of supracarinal and subcarinal low-flow oxygen insufflation to conventional intermittent positive-pressure ventilation ( IPPV ) of critically ill and anesthetized patients results in increased ventilation and improved oxygenation .
	manualset3
161644	8	411921	7	NULL	NULL	NULL	NULL	increased ventilation 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether the addition of supracarinal and subcarinal low-flow oxygen insufflation to conventional intermittent positive-pressure ventilation ( IPPV ) of critically ill and anesthetized patients results in increased ventilation and improved oxygenation .
	manualset3
161645	9	411921	7	NULL	NULL	NULL	NULL	 improved oxygenation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to determine whether the addition of supracarinal and subcarinal low-flow oxygen insufflation to conventional intermittent positive-pressure ventilation ( IPPV ) of critically ill and anesthetized patients results in increased ventilation and improved oxygenation .
	manualset3
161646	1	411922	7	NULL	NULL	0	NULL	Abdominal pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Abdominal pain and two x-rays : spot the difference .
	manualset3
161647	2	411922	7	NULL	NULL	0	NULL	 x-rays	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Abdominal pain and two x-rays : spot the difference .
	manualset3
169461	3	411922	7	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Abdominal pain and two x-rays : spot the difference .
	manualset3
161648	1	411923	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to evaluate the activity of digastric , sternocleidomastoid , upper trapezius , lower trapezius and cervical muscles in response to maximum voluntary clenching ( MVC ) of the teeth .
	manualset3
161649	2	411923	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to evaluate the activity of digastric , sternocleidomastoid , upper trapezius , lower trapezius and cervical muscles in response to maximum voluntary clenching ( MVC ) of the teeth .
	manualset3
161650	3	411923	7	NULL	NULL	0	NULL	digastric muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to evaluate the activity of digastric , sternocleidomastoid , upper trapezius , lower trapezius and cervical muscles in response to maximum voluntary clenching ( MVC ) of the teeth .
	manualset3
161651	4	411923	7	NULL	NULL	0	NULL	 sternocleidomastoid muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to evaluate the activity of digastric , sternocleidomastoid , upper trapezius , lower trapezius and cervical muscles in response to maximum voluntary clenching ( MVC ) of the teeth .
	manualset3
161652	5	411923	7	NULL	NULL	0	NULL	upper trapezius muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to evaluate the activity of digastric , sternocleidomastoid , upper trapezius , lower trapezius and cervical muscles in response to maximum voluntary clenching ( MVC ) of the teeth .
	manualset3
161653	6	411923	7	NULL	NULL	0	NULL	lower trapezius muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to evaluate the activity of digastric , sternocleidomastoid , upper trapezius , lower trapezius and cervical muscles in response to maximum voluntary clenching ( MVC ) of the teeth .
	manualset3
161654	7	411923	7	NULL	NULL	0	NULL	cervical muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to evaluate the activity of digastric , sternocleidomastoid , upper trapezius , lower trapezius and cervical muscles in response to maximum voluntary clenching ( MVC ) of the teeth .
	manualset3
161655	8	411923	7	NULL	NULL	0	NULL	maximum voluntary clenching ( MVC )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to evaluate the activity of digastric , sternocleidomastoid , upper trapezius , lower trapezius and cervical muscles in response to maximum voluntary clenching ( MVC ) of the teeth .
	manualset3
161656	9	411923	7	NULL	NULL	0	NULL	 teeth	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to evaluate the activity of digastric , sternocleidomastoid , upper trapezius , lower trapezius and cervical muscles in response to maximum voluntary clenching ( MVC ) of the teeth .
	manualset3
162361	10	411923	7	NULL	NULL	0	NULL	activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to evaluate the activity of digastric , sternocleidomastoid , upper trapezius , lower trapezius and cervical muscles in response to maximum voluntary clenching ( MVC ) of the teeth .
	manualset3
162508	11	411923	7	NULL	NULL	0	NULL	response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to evaluate the activity of digastric , sternocleidomastoid , upper trapezius , lower trapezius and cervical muscles in response to maximum voluntary clenching ( MVC ) of the teeth .
	manualset3
161657	1	411924	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to evaluate the killing effect that treatment in gravity or high-vacuum steam autoclaves had on endospores present on strips or applied to dental needles within 10 types of small sharps containers .
	manualset3
161658	2	411924	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to evaluate the killing effect that treatment in gravity or high-vacuum steam autoclaves had on endospores present on strips or applied to dental needles within 10 types of small sharps containers .
	manualset3
161659	3	411924	7	NULL	NULL	0	NULL	killing effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to evaluate the killing effect that treatment in gravity or high-vacuum steam autoclaves had on endospores present on strips or applied to dental needles within 10 types of small sharps containers .
	manualset3
161660	4	411924	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to evaluate the killing effect that treatment in gravity or high-vacuum steam autoclaves had on endospores present on strips or applied to dental needles within 10 types of small sharps containers .
	manualset3
161661	5	411924	7	NULL	NULL	0	NULL	gravity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to evaluate the killing effect that treatment in gravity or high-vacuum steam autoclaves had on endospores present on strips or applied to dental needles within 10 types of small sharps containers .
	manualset3
161662	6	411924	7	NULL	NULL	0	NULL	high-vacuum steam autoclaves	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to evaluate the killing effect that treatment in gravity or high-vacuum steam autoclaves had on endospores present on strips or applied to dental needles within 10 types of small sharps containers .
	manualset3
161663	7	411924	7	NULL	NULL	0	NULL	endospores	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to evaluate the killing effect that treatment in gravity or high-vacuum steam autoclaves had on endospores present on strips or applied to dental needles within 10 types of small sharps containers .
	manualset3
161664	8	411924	7	NULL	NULL	0	NULL	strips	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to evaluate the killing effect that treatment in gravity or high-vacuum steam autoclaves had on endospores present on strips or applied to dental needles within 10 types of small sharps containers .
	manualset3
161665	9	411924	7	NULL	NULL	0	NULL	dental needles	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to evaluate the killing effect that treatment in gravity or high-vacuum steam autoclaves had on endospores present on strips or applied to dental needles within 10 types of small sharps containers .
	manualset3
161666	10	411924	7	NULL	NULL	0	NULL	10 types 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to evaluate the killing effect that treatment in gravity or high-vacuum steam autoclaves had on endospores present on strips or applied to dental needles within 10 types of small sharps containers .
	manualset3
161667	11	411924	7	NULL	NULL	0	NULL	small sharps containers	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to evaluate the killing effect that treatment in gravity or high-vacuum steam autoclaves had on endospores present on strips or applied to dental needles within 10 types of small sharps containers .
	manualset3
161668	1	411925	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to examine the effects of COX-2 deficiency on neuronal vulnerability after transient forebrain ischemia .
	manualset3
161669	2	411925	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to examine the effects of COX-2 deficiency on neuronal vulnerability after transient forebrain ischemia .
	manualset3
161670	3	411925	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to examine the effects of COX-2 deficiency on neuronal vulnerability after transient forebrain ischemia .
	manualset3
161671	4	411925	7	NULL	NULL	0	NULL	COX-2 deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to examine the effects of COX-2 deficiency on neuronal vulnerability after transient forebrain ischemia .
	manualset3
161672	5	411925	7	NULL	NULL	0	NULL	neuronal vulnerability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to examine the effects of COX-2 deficiency on neuronal vulnerability after transient forebrain ischemia .
	manualset3
161673	6	411925	7	NULL	NULL	0	NULL	transient forebrain ischemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to examine the effects of COX-2 deficiency on neuronal vulnerability after transient forebrain ischemia .
	manualset3
161674	1	411926	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to examine the pattern of inheritance in a large number of families in an attempt to find clues to pathogenesis .
	manualset3
161675	2	411926	7	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to examine the pattern of inheritance in a large number of families in an attempt to find clues to pathogenesis .
	manualset3
161676	3	411926	7	NULL	NULL	0	NULL	pattern of inheritance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to examine the pattern of inheritance in a large number of families in an attempt to find clues to pathogenesis .
	manualset3
161677	4	411926	7	NULL	NULL	0	NULL	large number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to examine the pattern of inheritance in a large number of families in an attempt to find clues to pathogenesis .
	manualset3
161678	5	411926	7	NULL	NULL	0	NULL	 families	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to examine the pattern of inheritance in a large number of families in an attempt to find clues to pathogenesis .
	manualset3
161679	6	411926	7	NULL	NULL	0	NULL	clues	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to examine the pattern of inheritance in a large number of families in an attempt to find clues to pathogenesis .
	manualset3
161680	7	411926	7	NULL	NULL	0	NULL	pathogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to examine the pattern of inheritance in a large number of families in an attempt to find clues to pathogenesis .
	manualset3
169462	8	411926	7	NULL	NULL	0	NULL	attempt	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to examine the pattern of inheritance in a large number of families in an attempt to find clues to pathogenesis .
	manualset3
161681	1	411927	7	NULL	NULL	0	NULL	 purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate signaling and regulatory mechanisms of apoptosis in a model of focal and segmental glomerulosclerosis .
	manualset3
161682	2	411927	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate signaling and regulatory mechanisms of apoptosis in a model of focal and segmental glomerulosclerosis .
	manualset3
161683	3	411927	7	NULL	NULL	0	NULL	 signaling and regulatory mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate signaling and regulatory mechanisms of apoptosis in a model of focal and segmental glomerulosclerosis .
	manualset3
161684	4	411927	7	NULL	NULL	0	NULL	apoptosis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate signaling and regulatory mechanisms of apoptosis in a model of focal and segmental glomerulosclerosis .
	manualset3
161685	5	411927	7	NULL	NULL	0	NULL	focal glomerulosclerosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate signaling and regulatory mechanisms of apoptosis in a model of focal and segmental glomerulosclerosis .
	manualset3
161686	6	411927	7	NULL	NULL	0	NULL	segmental glomerulosclerosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate signaling and regulatory mechanisms of apoptosis in a model of focal and segmental glomerulosclerosis .
	manualset3
161687	7	411927	7	NULL	NULL	0	NULL	model	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate signaling and regulatory mechanisms of apoptosis in a model of focal and segmental glomerulosclerosis .
	manualset3
161688	1	411928	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate the effectiveness of intermittent pneumatic compression of the plantar venous plexus with the newly developed arteriovenous impulse system .
	manualset3
161689	2	411928	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate the effectiveness of intermittent pneumatic compression of the plantar venous plexus with the newly developed arteriovenous impulse system .
	manualset3
161690	3	411928	7	NULL	NULL	0	NULL	intermittent pneumatic compression	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate the effectiveness of intermittent pneumatic compression of the plantar venous plexus with the newly developed arteriovenous impulse system .
	manualset3
161691	4	411928	7	NULL	NULL	0	NULL	plantar venous plexus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate the effectiveness of intermittent pneumatic compression of the plantar venous plexus with the newly developed arteriovenous impulse system .
	manualset3
161692	5	411928	7	NULL	NULL	0	NULL	arteriovenous impulse system	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate the effectiveness of intermittent pneumatic compression of the plantar venous plexus with the newly developed arteriovenous impulse system .
	manualset3
169463	6	411928	7	NULL	NULL	0	NULL	 effectiveness 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate the effectiveness of intermittent pneumatic compression of the plantar venous plexus with the newly developed arteriovenous impulse system .
	manualset3
161693	1	411929	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate the possible existence of systematic differences between moment-length properties of the rectus femoris muscle of cyclists/speed skaters and runners .
	manualset3
161694	2	411929	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate the possible existence of systematic differences between moment-length properties of the rectus femoris muscle of cyclists/speed skaters and runners .
	manualset3
161695	3	411929	7	NULL	NULL	0	NULL	 existence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate the possible existence of systematic differences between moment-length properties of the rectus femoris muscle of cyclists/speed skaters and runners .
	manualset3
161696	4	411929	7	NULL	NULL	0	NULL	moment-length properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate the possible existence of systematic differences between moment-length properties of the rectus femoris muscle of cyclists/speed skaters and runners .
	manualset3
161697	5	411929	7	NULL	NULL	0	NULL	rectus femoris muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate the possible existence of systematic differences between moment-length properties of the rectus femoris muscle of cyclists/speed skaters and runners .
	manualset3
161698	6	411929	7	NULL	NULL	0	NULL	cyclists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate the possible existence of systematic differences between moment-length properties of the rectus femoris muscle of cyclists/speed skaters and runners .
	manualset3
161699	7	411929	7	NULL	NULL	0	NULL	speed skaters	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate the possible existence of systematic differences between moment-length properties of the rectus femoris muscle of cyclists/speed skaters and runners .
	manualset3
161700	8	411929	7	NULL	NULL	0	NULL	runners	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate the possible existence of systematic differences between moment-length properties of the rectus femoris muscle of cyclists/speed skaters and runners .
	manualset3
169464	9	411929	7	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate the possible existence of systematic differences between moment-length properties of the rectus femoris muscle of cyclists/speed skaters and runners .
	manualset3
161701	1	411930	7	NULL	NULL	0	NULL	Abdominal pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Abdominal pain is relieved after a bizarre GI finding .
	manualset3
161702	2	411930	7	NULL	NULL	0	NULL	GI finding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Abdominal pain is relieved after a bizarre GI finding .
	manualset3
161708	1	411931	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate whether dental injury diagnoses may predict adverse outcomes occurring 102 weeks after trauma , and to evaluate whether the severity of adverse outcome is related to laser Doppler flowmetry ( LDF ) measurements of blood flow from teeth .
	manualset3
161709	2	411931	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate whether dental injury diagnoses may predict adverse outcomes occurring 102 weeks after trauma , and to evaluate whether the severity of adverse outcome is related to laser Doppler flowmetry ( LDF ) measurements of blood flow from teeth .
	manualset3
161710	3	411931	7	NULL	NULL	0	NULL	dental injury diagnoses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate whether dental injury diagnoses may predict adverse outcomes occurring 102 weeks after trauma , and to evaluate whether the severity of adverse outcome is related to laser Doppler flowmetry ( LDF ) measurements of blood flow from teeth .
	manualset3
161711	4	411931	7	NULL	NULL	0	NULL	adverse outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate whether dental injury diagnoses may predict adverse outcomes occurring 102 weeks after trauma , and to evaluate whether the severity of adverse outcome is related to laser Doppler flowmetry ( LDF ) measurements of blood flow from teeth .
	manualset3
161712	5	411931	7	NULL	NULL	0	NULL	102 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate whether dental injury diagnoses may predict adverse outcomes occurring 102 weeks after trauma , and to evaluate whether the severity of adverse outcome is related to laser Doppler flowmetry ( LDF ) measurements of blood flow from teeth .
	manualset3
161713	6	411931	7	NULL	NULL	0	NULL	 trauma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate whether dental injury diagnoses may predict adverse outcomes occurring 102 weeks after trauma , and to evaluate whether the severity of adverse outcome is related to laser Doppler flowmetry ( LDF ) measurements of blood flow from teeth .
	manualset3
161714	7	411931	7	NULL	NULL	0	NULL	adverse outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate whether dental injury diagnoses may predict adverse outcomes occurring 102 weeks after trauma , and to evaluate whether the severity of adverse outcome is related to laser Doppler flowmetry ( LDF ) measurements of blood flow from teeth .
	manualset3
161715	8	411931	7	NULL	NULL	0	NULL	laser Doppler flowmetry ( LDF ) measurements	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate whether dental injury diagnoses may predict adverse outcomes occurring 102 weeks after trauma , and to evaluate whether the severity of adverse outcome is related to laser Doppler flowmetry ( LDF ) measurements of blood flow from teeth .
	manualset3
161716	9	411931	7	NULL	NULL	0	NULL	blood flow	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate whether dental injury diagnoses may predict adverse outcomes occurring 102 weeks after trauma , and to evaluate whether the severity of adverse outcome is related to laser Doppler flowmetry ( LDF ) measurements of blood flow from teeth .
	manualset3
161717	10	411931	7	NULL	NULL	0	NULL	teeth	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate whether dental injury diagnoses may predict adverse outcomes occurring 102 weeks after trauma , and to evaluate whether the severity of adverse outcome is related to laser Doppler flowmetry ( LDF ) measurements of blood flow from teeth .
	manualset3
162348	11	411931	7	NULL	NULL	0	NULL	severity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to investigate whether dental injury diagnoses may predict adverse outcomes occurring 102 weeks after trauma , and to evaluate whether the severity of adverse outcome is related to laser Doppler flowmetry ( LDF ) measurements of blood flow from teeth .
	manualset3
161718	1	411932	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to use our established partial patellectomy rabbit model to study the effects of low-intensity pulsed ultrasound ( LIPUS ) on patella-patellar tendon ( PPT ) junction repair through hypothesized pathways including regulation of vascular endothelial growth factor ( VEGF ) and chondrogenesis .
	manualset3
161719	2	411932	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to use our established partial patellectomy rabbit model to study the effects of low-intensity pulsed ultrasound ( LIPUS ) on patella-patellar tendon ( PPT ) junction repair through hypothesized pathways including regulation of vascular endothelial growth factor ( VEGF ) and chondrogenesis .
	manualset3
161720	3	411932	7	NULL	NULL	NULL	NULL	partial patellectomy rabbit model	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to use our established partial patellectomy rabbit model to study the effects of low-intensity pulsed ultrasound ( LIPUS ) on patella-patellar tendon ( PPT ) junction repair through hypothesized pathways including regulation of vascular endothelial growth factor ( VEGF ) and chondrogenesis .
	manualset3
161722	5	411932	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to use our established partial patellectomy rabbit model to study the effects of low-intensity pulsed ultrasound ( LIPUS ) on patella-patellar tendon ( PPT ) junction repair through hypothesized pathways including regulation of vascular endothelial growth factor ( VEGF ) and chondrogenesis .
	manualset3
161723	6	411932	7	NULL	NULL	0	NULL	low-intensity pulsed ultrasound ( LIPUS )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to use our established partial patellectomy rabbit model to study the effects of low-intensity pulsed ultrasound ( LIPUS ) on patella-patellar tendon ( PPT ) junction repair through hypothesized pathways including regulation of vascular endothelial growth factor ( VEGF ) and chondrogenesis .
	manualset3
161724	7	411932	7	NULL	NULL	NULL	NULL	patella-patellar tendon ( PPT ) junction repair	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to use our established partial patellectomy rabbit model to study the effects of low-intensity pulsed ultrasound ( LIPUS ) on patella-patellar tendon ( PPT ) junction repair through hypothesized pathways including regulation of vascular endothelial growth factor ( VEGF ) and chondrogenesis .
	manualset3
161725	8	411932	7	NULL	NULL	0	NULL	hypothesized pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to use our established partial patellectomy rabbit model to study the effects of low-intensity pulsed ultrasound ( LIPUS ) on patella-patellar tendon ( PPT ) junction repair through hypothesized pathways including regulation of vascular endothelial growth factor ( VEGF ) and chondrogenesis .
	manualset3
161726	9	411932	7	NULL	NULL	0	NULL	 regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to use our established partial patellectomy rabbit model to study the effects of low-intensity pulsed ultrasound ( LIPUS ) on patella-patellar tendon ( PPT ) junction repair through hypothesized pathways including regulation of vascular endothelial growth factor ( VEGF ) and chondrogenesis .
	manualset3
161727	10	411932	7	NULL	NULL	0	NULL	vascular endothelial growth factor ( VEGF )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to use our established partial patellectomy rabbit model to study the effects of low-intensity pulsed ultrasound ( LIPUS ) on patella-patellar tendon ( PPT ) junction repair through hypothesized pathways including regulation of vascular endothelial growth factor ( VEGF ) and chondrogenesis .
	manualset3
161728	11	411932	7	NULL	NULL	0	NULL	chondrogenesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this study was to use our established partial patellectomy rabbit model to study the effects of low-intensity pulsed ultrasound ( LIPUS ) on patella-patellar tendon ( PPT ) junction repair through hypothesized pathways including regulation of vascular endothelial growth factor ( VEGF ) and chondrogenesis .
	manualset3
161729	1	411933	7	NULL	NULL	0	NULL	purpose	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose was to characterize the family goals of survival , continuity , and growth from the parental perspective during early family formation .
	manualset3
161730	2	411933	7	NULL	NULL	NULL	NULL	family goals 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose was to characterize the family goals of survival , continuity , and growth from the parental perspective during early family formation .
	manualset3
161731	3	411933	7	NULL	NULL	0	NULL	continuity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose was to characterize the family goals of survival , continuity , and growth from the parental perspective during early family formation .
	manualset3
161732	4	411933	7	NULL	NULL	0	NULL	growth	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose was to characterize the family goals of survival , continuity , and growth from the parental perspective during early family formation .
	manualset3
161733	5	411933	7	NULL	NULL	0	NULL	parental perspective	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose was to characterize the family goals of survival , continuity , and growth from the parental perspective during early family formation .
	manualset3
161734	6	411933	7	NULL	NULL	0	NULL	 early family formation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose was to characterize the family goals of survival , continuity , and growth from the parental perspective during early family formation .
	manualset3
162349	7	411933	7	NULL	NULL	0	NULL	survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose was to characterize the family goals of survival , continuity , and growth from the parental perspective during early family formation .
	manualset3
161735	1	411934	7	NULL	NULL	0	NULL	purpose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose was to introduce a novel method for computer-based classification of visual field data derived from perimetric examination , that may act as a ` counsellor ' , providing an independent ` second opinion ' to the diagnosing physician .
	manualset3
161736	2	411934	7	NULL	NULL	0	NULL	novel method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose was to introduce a novel method for computer-based classification of visual field data derived from perimetric examination , that may act as a ` counsellor ' , providing an independent ` second opinion ' to the diagnosing physician .
	manualset3
161737	3	411934	7	NULL	NULL	0	NULL	computer-based classification 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose was to introduce a novel method for computer-based classification of visual field data derived from perimetric examination , that may act as a ` counsellor ' , providing an independent ` second opinion ' to the diagnosing physician .
	manualset3
161738	4	411934	7	NULL	NULL	0	NULL	visual field data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose was to introduce a novel method for computer-based classification of visual field data derived from perimetric examination , that may act as a ` counsellor ' , providing an independent ` second opinion ' to the diagnosing physician .
	manualset3
161739	5	411934	7	NULL	NULL	0	NULL	perimetric examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose was to introduce a novel method for computer-based classification of visual field data derived from perimetric examination , that may act as a ` counsellor ' , providing an independent ` second opinion ' to the diagnosing physician .
	manualset3
161740	6	411934	7	NULL	NULL	0	NULL	counsellor	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose was to introduce a novel method for computer-based classification of visual field data derived from perimetric examination , that may act as a ` counsellor ' , providing an independent ` second opinion ' to the diagnosing physician .
	manualset3
161741	7	411934	7	NULL	NULL	NULL	NULL	second opinion	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose was to introduce a novel method for computer-based classification of visual field data derived from perimetric examination , that may act as a ` counsellor ' , providing an independent ` second opinion ' to the diagnosing physician .
	manualset3
161742	8	411934	7	NULL	NULL	NULL	NULL	diagnosing physician	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose was to introduce a novel method for computer-based classification of visual field data derived from perimetric examination , that may act as a ` counsellor ' , providing an independent ` second opinion ' to the diagnosing physician .
	manualset3
161743	1	411935	7	NULL	NULL	0	NULL	 purposes	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purposes of the current study were : ( 1 ) to investigate the immunoregulatory effects of T-cell growth factor ( TCGF ) on the activation and differentiation of syngeneic cytotoxic T lymphocyte ( CTL ) populations generated against a 20-methylcholanthrene-induced ependymoblastoma , 203-glioma , in C57BL/6 mice ; and ( 2 ) to determine whether the glioma-specific CTL clone ( G-CTLL ) could be established by TCGF , and whether the in vivo efficacy of the cloned cells could be rendered more effective in adoptive therapy .
	manualset3
161744	2	411935	7	NULL	NULL	0	NULL	current study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purposes of the current study were : ( 1 ) to investigate the immunoregulatory effects of T-cell growth factor ( TCGF ) on the activation and differentiation of syngeneic cytotoxic T lymphocyte ( CTL ) populations generated against a 20-methylcholanthrene-induced ependymoblastoma , 203-glioma , in C57BL/6 mice ; and ( 2 ) to determine whether the glioma-specific CTL clone ( G-CTLL ) could be established by TCGF , and whether the in vivo efficacy of the cloned cells could be rendered more effective in adoptive therapy .
	manualset3
161745	3	411935	7	NULL	NULL	0	NULL	immunoregulatory effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purposes of the current study were : ( 1 ) to investigate the immunoregulatory effects of T-cell growth factor ( TCGF ) on the activation and differentiation of syngeneic cytotoxic T lymphocyte ( CTL ) populations generated against a 20-methylcholanthrene-induced ependymoblastoma , 203-glioma , in C57BL/6 mice ; and ( 2 ) to determine whether the glioma-specific CTL clone ( G-CTLL ) could be established by TCGF , and whether the in vivo efficacy of the cloned cells could be rendered more effective in adoptive therapy .
	manualset3
161746	4	411935	7	NULL	NULL	0	NULL	T-cell growth factor ( TCGF )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The purposes of the current study were : ( 1 ) to investigate the immunoregulatory effects of T-cell growth factor ( TCGF ) on the activation and differentiation of syngeneic cytotoxic T lymphocyte ( CTL ) populations generated against a 20-methylcholanthrene-induced ependymoblastoma , 203-glioma , in C57BL/6 mice ; and ( 2 ) to determine whether the glioma-specific CTL clone ( G-CTLL ) could be established by TCGF , and whether the in vivo efficacy of the cloned cells could be rendered more effective in adoptive therapy .
	manualset3
161747	5	411935	7	NULL	NULL	0	NULL	activation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purposes of the current study were : ( 1 ) to investigate the immunoregulatory effects of T-cell growth factor ( TCGF ) on the activation and differentiation of syngeneic cytotoxic T lymphocyte ( CTL ) populations generated against a 20-methylcholanthrene-induced ependymoblastoma , 203-glioma , in C57BL/6 mice ; and ( 2 ) to determine whether the glioma-specific CTL clone ( G-CTLL ) could be established by TCGF , and whether the in vivo efficacy of the cloned cells could be rendered more effective in adoptive therapy .
	manualset3
161748	6	411935	7	NULL	NULL	0	NULL	differentiation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purposes of the current study were : ( 1 ) to investigate the immunoregulatory effects of T-cell growth factor ( TCGF ) on the activation and differentiation of syngeneic cytotoxic T lymphocyte ( CTL ) populations generated against a 20-methylcholanthrene-induced ependymoblastoma , 203-glioma , in C57BL/6 mice ; and ( 2 ) to determine whether the glioma-specific CTL clone ( G-CTLL ) could be established by TCGF , and whether the in vivo efficacy of the cloned cells could be rendered more effective in adoptive therapy .
	manualset3
161749	7	411935	7	NULL	NULL	0	NULL	syngeneic cytotoxic T lymphocyte ( CTL ) populations	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The purposes of the current study were : ( 1 ) to investigate the immunoregulatory effects of T-cell growth factor ( TCGF ) on the activation and differentiation of syngeneic cytotoxic T lymphocyte ( CTL ) populations generated against a 20-methylcholanthrene-induced ependymoblastoma , 203-glioma , in C57BL/6 mice ; and ( 2 ) to determine whether the glioma-specific CTL clone ( G-CTLL ) could be established by TCGF , and whether the in vivo efficacy of the cloned cells could be rendered more effective in adoptive therapy .
	manualset3
161750	8	411935	7	NULL	NULL	0	NULL	20-methylcholanthrene-induced ependymoblastoma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purposes of the current study were : ( 1 ) to investigate the immunoregulatory effects of T-cell growth factor ( TCGF ) on the activation and differentiation of syngeneic cytotoxic T lymphocyte ( CTL ) populations generated against a 20-methylcholanthrene-induced ependymoblastoma , 203-glioma , in C57BL/6 mice ; and ( 2 ) to determine whether the glioma-specific CTL clone ( G-CTLL ) could be established by TCGF , and whether the in vivo efficacy of the cloned cells could be rendered more effective in adoptive therapy .
	manualset3
161751	9	411935	7	NULL	NULL	0	NULL	203-glioma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purposes of the current study were : ( 1 ) to investigate the immunoregulatory effects of T-cell growth factor ( TCGF ) on the activation and differentiation of syngeneic cytotoxic T lymphocyte ( CTL ) populations generated against a 20-methylcholanthrene-induced ependymoblastoma , 203-glioma , in C57BL/6 mice ; and ( 2 ) to determine whether the glioma-specific CTL clone ( G-CTLL ) could be established by TCGF , and whether the in vivo efficacy of the cloned cells could be rendered more effective in adoptive therapy .
	manualset3
161752	10	411935	7	NULL	NULL	0	NULL	C57BL/6 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The purposes of the current study were : ( 1 ) to investigate the immunoregulatory effects of T-cell growth factor ( TCGF ) on the activation and differentiation of syngeneic cytotoxic T lymphocyte ( CTL ) populations generated against a 20-methylcholanthrene-induced ependymoblastoma , 203-glioma , in C57BL/6 mice ; and ( 2 ) to determine whether the glioma-specific CTL clone ( G-CTLL ) could be established by TCGF , and whether the in vivo efficacy of the cloned cells could be rendered more effective in adoptive therapy .
	manualset3
161753	11	411935	7	NULL	NULL	0	NULL	glioma-specific CTL clone ( G-CTLL )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The purposes of the current study were : ( 1 ) to investigate the immunoregulatory effects of T-cell growth factor ( TCGF ) on the activation and differentiation of syngeneic cytotoxic T lymphocyte ( CTL ) populations generated against a 20-methylcholanthrene-induced ependymoblastoma , 203-glioma , in C57BL/6 mice ; and ( 2 ) to determine whether the glioma-specific CTL clone ( G-CTLL ) could be established by TCGF , and whether the in vivo efficacy of the cloned cells could be rendered more effective in adoptive therapy .
	manualset3
161754	12	411935	7	NULL	NULL	0	NULL	TCGF 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The purposes of the current study were : ( 1 ) to investigate the immunoregulatory effects of T-cell growth factor ( TCGF ) on the activation and differentiation of syngeneic cytotoxic T lymphocyte ( CTL ) populations generated against a 20-methylcholanthrene-induced ependymoblastoma , 203-glioma , in C57BL/6 mice ; and ( 2 ) to determine whether the glioma-specific CTL clone ( G-CTLL ) could be established by TCGF , and whether the in vivo efficacy of the cloned cells could be rendered more effective in adoptive therapy .
	manualset3
161755	13	411935	7	NULL	NULL	0	NULL	cloned cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The purposes of the current study were : ( 1 ) to investigate the immunoregulatory effects of T-cell growth factor ( TCGF ) on the activation and differentiation of syngeneic cytotoxic T lymphocyte ( CTL ) populations generated against a 20-methylcholanthrene-induced ependymoblastoma , 203-glioma , in C57BL/6 mice ; and ( 2 ) to determine whether the glioma-specific CTL clone ( G-CTLL ) could be established by TCGF , and whether the in vivo efficacy of the cloned cells could be rendered more effective in adoptive therapy .
	manualset3
161756	14	411935	7	NULL	NULL	0	NULL	adoptive therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The purposes of the current study were : ( 1 ) to investigate the immunoregulatory effects of T-cell growth factor ( TCGF ) on the activation and differentiation of syngeneic cytotoxic T lymphocyte ( CTL ) populations generated against a 20-methylcholanthrene-induced ependymoblastoma , 203-glioma , in C57BL/6 mice ; and ( 2 ) to determine whether the glioma-specific CTL clone ( G-CTLL ) could be established by TCGF , and whether the in vivo efficacy of the cloned cells could be rendered more effective in adoptive therapy .
	manualset3
169465	15	411935	7	NULL	NULL	0	NULL	in vivo efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purposes of the current study were : ( 1 ) to investigate the immunoregulatory effects of T-cell growth factor ( TCGF ) on the activation and differentiation of syngeneic cytotoxic T lymphocyte ( CTL ) populations generated against a 20-methylcholanthrene-induced ependymoblastoma , 203-glioma , in C57BL/6 mice ; and ( 2 ) to determine whether the glioma-specific CTL clone ( G-CTLL ) could be established by TCGF , and whether the in vivo efficacy of the cloned cells could be rendered more effective in adoptive therapy .
	manualset3
161757	1	411936	7	NULL	NULL	0	NULL	purposes	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purposes of this research were to first examine the evidence regarding the factor structure of educational achievement tests in the context of two theoretical models of cognitive ability ( psychometric g and mutualism ) that have been proposed to explain this structure as well as the underlying processes that may be responsible for its emergence in dimensionality studies .
	manualset3
161758	2	411936	7	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purposes of this research were to first examine the evidence regarding the factor structure of educational achievement tests in the context of two theoretical models of cognitive ability ( psychometric g and mutualism ) that have been proposed to explain this structure as well as the underlying processes that may be responsible for its emergence in dimensionality studies .
	manualset3
161759	3	411936	7	NULL	NULL	0	NULL	 evidence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purposes of this research were to first examine the evidence regarding the factor structure of educational achievement tests in the context of two theoretical models of cognitive ability ( psychometric g and mutualism ) that have been proposed to explain this structure as well as the underlying processes that may be responsible for its emergence in dimensionality studies .
	manualset3
161760	4	411936	7	NULL	NULL	0	NULL	factor structure 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purposes of this research were to first examine the evidence regarding the factor structure of educational achievement tests in the context of two theoretical models of cognitive ability ( psychometric g and mutualism ) that have been proposed to explain this structure as well as the underlying processes that may be responsible for its emergence in dimensionality studies .
	manualset3
161761	5	411936	7	NULL	NULL	0	NULL	educational achievement tests 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purposes of this research were to first examine the evidence regarding the factor structure of educational achievement tests in the context of two theoretical models of cognitive ability ( psychometric g and mutualism ) that have been proposed to explain this structure as well as the underlying processes that may be responsible for its emergence in dimensionality studies .
	manualset3
161762	6	411936	7	NULL	NULL	0	NULL	context 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purposes of this research were to first examine the evidence regarding the factor structure of educational achievement tests in the context of two theoretical models of cognitive ability ( psychometric g and mutualism ) that have been proposed to explain this structure as well as the underlying processes that may be responsible for its emergence in dimensionality studies .
	manualset3
161763	7	411936	7	NULL	NULL	NULL	NULL	theoretical models of cognitive ability	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purposes of this research were to first examine the evidence regarding the factor structure of educational achievement tests in the context of two theoretical models of cognitive ability ( psychometric g and mutualism ) that have been proposed to explain this structure as well as the underlying processes that may be responsible for its emergence in dimensionality studies .
	manualset3
161764	8	411936	7	NULL	NULL	NULL	NULL	psychometric g	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purposes of this research were to first examine the evidence regarding the factor structure of educational achievement tests in the context of two theoretical models of cognitive ability ( psychometric g and mutualism ) that have been proposed to explain this structure as well as the underlying processes that may be responsible for its emergence in dimensionality studies .
	manualset3
161765	9	411936	7	NULL	NULL	NULL	NULL	mutualism	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purposes of this research were to first examine the evidence regarding the factor structure of educational achievement tests in the context of two theoretical models of cognitive ability ( psychometric g and mutualism ) that have been proposed to explain this structure as well as the underlying processes that may be responsible for its emergence in dimensionality studies .
	manualset3
161766	10	411936	7	NULL	NULL	0	NULL	structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purposes of this research were to first examine the evidence regarding the factor structure of educational achievement tests in the context of two theoretical models of cognitive ability ( psychometric g and mutualism ) that have been proposed to explain this structure as well as the underlying processes that may be responsible for its emergence in dimensionality studies .
	manualset3
161767	11	411936	7	NULL	NULL	0	NULL	processes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purposes of this research were to first examine the evidence regarding the factor structure of educational achievement tests in the context of two theoretical models of cognitive ability ( psychometric g and mutualism ) that have been proposed to explain this structure as well as the underlying processes that may be responsible for its emergence in dimensionality studies .
	manualset3
161768	13	411936	7	NULL	NULL	NULL	NULL	dimensionality studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purposes of this research were to first examine the evidence regarding the factor structure of educational achievement tests in the context of two theoretical models of cognitive ability ( psychometric g and mutualism ) that have been proposed to explain this structure as well as the underlying processes that may be responsible for its emergence in dimensionality studies .
	manualset3
162350	12	411936	7	NULL	NULL	NULL	NULL	emergence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purposes of this research were to first examine the evidence regarding the factor structure of educational achievement tests in the context of two theoretical models of cognitive ability ( psychometric g and mutualism ) that have been proposed to explain this structure as well as the underlying processes that may be responsible for its emergence in dimensionality studies .
	manualset3
161769	1	411937	7	NULL	NULL	NULL	NULL	quantification	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The quantification of DeltaR2 ( * ) under brain activation : dependence on relaxation rate at rest and significance threshold .
	manualset3
161770	2	411937	7	NULL	NULL	NULL	NULL	DeltaR2 ( * )	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The quantification of DeltaR2 ( * ) under brain activation : dependence on relaxation rate at rest and significance threshold .
	manualset3
161771	3	411937	7	NULL	NULL	0	NULL	brain activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The quantification of DeltaR2 ( * ) under brain activation : dependence on relaxation rate at rest and significance threshold .
	manualset3
161772	4	411937	7	NULL	NULL	0	NULL	 relaxation rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The quantification of DeltaR2 ( * ) under brain activation : dependence on relaxation rate at rest and significance threshold .
	manualset3
161773	5	411937	7	NULL	NULL	0	NULL	rest 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The quantification of DeltaR2 ( * ) under brain activation : dependence on relaxation rate at rest and significance threshold .
	manualset3
161774	6	411937	7	NULL	NULL	NULL	NULL	significance threshold	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The quantification of DeltaR2 ( * ) under brain activation : dependence on relaxation rate at rest and significance threshold .
	manualset3
161775	1	411938	7	NULL	NULL	0	NULL	 question	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The question is important both to our understanding of the biological mechanisms involved and for public health planning .
	manualset3
161776	2	411938	7	NULL	NULL	0	NULL	biological mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The question is important both to our understanding of the biological mechanisms involved and for public health planning .
	manualset3
161777	3	411938	7	NULL	NULL	NULL	NULL	public health planning	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The question is important both to our understanding of the biological mechanisms involved and for public health planning .
	manualset3
161778	1	411939	7	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Aberrant activation of the Wnt / - catenin signaling pathway is associated with a wide range of human cancers .
	manualset3
161779	2	411939	7	NULL	NULL	0	NULL	Wnt / - catenin signaling pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Aberrant activation of the Wnt / - catenin signaling pathway is associated with a wide range of human cancers .
	manualset3
161780	3	411939	7	NULL	NULL	0	NULL	human cancers	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Aberrant activation of the Wnt / - catenin signaling pathway is associated with a wide range of human cancers .
	manualset3
169466	4	411939	7	NULL	NULL	0	NULL	wide range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Aberrant activation of the Wnt / - catenin signaling pathway is associated with a wide range of human cancers .
	manualset3
161781	1	411940	7	NULL	NULL	NULL	NULL	 question 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The question of a possible association between prolonged early use of combined oral contraceptives ( COCs ) and an increased risk of breast cancer remains unresolved , despite the existence of at least 10 large-scale case-control studies and 5 large cohort studies .
	manualset3
161782	2	411940	7	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The question of a possible association between prolonged early use of combined oral contraceptives ( COCs ) and an increased risk of breast cancer remains unresolved , despite the existence of at least 10 large-scale case-control studies and 5 large cohort studies .
	manualset3
161783	3	411940	7	NULL	NULL	0	NULL	combined oral contraceptives ( COCs )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The question of a possible association between prolonged early use of combined oral contraceptives ( COCs ) and an increased risk of breast cancer remains unresolved , despite the existence of at least 10 large-scale case-control studies and 5 large cohort studies .
	manualset3
161784	4	411940	7	NULL	NULL	0	NULL	risk	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The question of a possible association between prolonged early use of combined oral contraceptives ( COCs ) and an increased risk of breast cancer remains unresolved , despite the existence of at least 10 large-scale case-control studies and 5 large cohort studies .
	manualset3
161785	5	411940	7	NULL	NULL	0	NULL	breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The question of a possible association between prolonged early use of combined oral contraceptives ( COCs ) and an increased risk of breast cancer remains unresolved , despite the existence of at least 10 large-scale case-control studies and 5 large cohort studies .
	manualset3
161786	6	411940	7	NULL	NULL	0	NULL	existence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The question of a possible association between prolonged early use of combined oral contraceptives ( COCs ) and an increased risk of breast cancer remains unresolved , despite the existence of at least 10 large-scale case-control studies and 5 large cohort studies .
	manualset3
161787	7	411940	7	NULL	NULL	0	NULL	 10 large-scale	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The question of a possible association between prolonged early use of combined oral contraceptives ( COCs ) and an increased risk of breast cancer remains unresolved , despite the existence of at least 10 large-scale case-control studies and 5 large cohort studies .
	manualset3
161788	8	411940	7	NULL	NULL	0	NULL	case-control studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The question of a possible association between prolonged early use of combined oral contraceptives ( COCs ) and an increased risk of breast cancer remains unresolved , despite the existence of at least 10 large-scale case-control studies and 5 large cohort studies .
	manualset3
161789	9	411940	7	NULL	NULL	0	NULL	5 large cohort studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The question of a possible association between prolonged early use of combined oral contraceptives ( COCs ) and an increased risk of breast cancer remains unresolved , despite the existence of at least 10 large-scale case-control studies and 5 large cohort studies .
	manualset3
169467	10	411940	7	NULL	NULL	0	NULL	prolonged early use	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The question of a possible association between prolonged early use of combined oral contraceptives ( COCs ) and an increased risk of breast cancer remains unresolved , despite the existence of at least 10 large-scale case-control studies and 5 large cohort studies .
	manualset3
161790	1	411941	7	NULL	NULL	0	NULL	question	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The question of a possible precursor -- product relationship between oval cells and hepatocytes was examined in rats treated for 2 weeks with 2-acetylaminofluorene ( 2-AAF ) with a two-thirds partial hepatectomy ( PH ) performed after the first week of 2-AAF treatment ( modified Solt-Farber model ) .
	manualset3
161791	2	411941	7	NULL	NULL	0	NULL	precursor -- product relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The question of a possible precursor -- product relationship between oval cells and hepatocytes was examined in rats treated for 2 weeks with 2-acetylaminofluorene ( 2-AAF ) with a two-thirds partial hepatectomy ( PH ) performed after the first week of 2-AAF treatment ( modified Solt-Farber model ) .
	manualset3
161792	3	411941	7	NULL	NULL	0	NULL	oval cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The question of a possible precursor -- product relationship between oval cells and hepatocytes was examined in rats treated for 2 weeks with 2-acetylaminofluorene ( 2-AAF ) with a two-thirds partial hepatectomy ( PH ) performed after the first week of 2-AAF treatment ( modified Solt-Farber model ) .
	manualset3
161793	4	411941	7	NULL	NULL	0	NULL	hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The question of a possible precursor -- product relationship between oval cells and hepatocytes was examined in rats treated for 2 weeks with 2-acetylaminofluorene ( 2-AAF ) with a two-thirds partial hepatectomy ( PH ) performed after the first week of 2-AAF treatment ( modified Solt-Farber model ) .
	manualset3
161794	5	411941	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The question of a possible precursor -- product relationship between oval cells and hepatocytes was examined in rats treated for 2 weeks with 2-acetylaminofluorene ( 2-AAF ) with a two-thirds partial hepatectomy ( PH ) performed after the first week of 2-AAF treatment ( modified Solt-Farber model ) .
	manualset3
161795	6	411941	7	NULL	NULL	0	NULL	2 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The question of a possible precursor -- product relationship between oval cells and hepatocytes was examined in rats treated for 2 weeks with 2-acetylaminofluorene ( 2-AAF ) with a two-thirds partial hepatectomy ( PH ) performed after the first week of 2-AAF treatment ( modified Solt-Farber model ) .
	manualset3
161796	7	411941	7	NULL	NULL	0	NULL	2-acetylaminofluorene ( 2-AAF )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The question of a possible precursor -- product relationship between oval cells and hepatocytes was examined in rats treated for 2 weeks with 2-acetylaminofluorene ( 2-AAF ) with a two-thirds partial hepatectomy ( PH ) performed after the first week of 2-AAF treatment ( modified Solt-Farber model ) .
	manualset3
161797	8	411941	7	NULL	NULL	0	NULL	two-thirds	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The question of a possible precursor -- product relationship between oval cells and hepatocytes was examined in rats treated for 2 weeks with 2-acetylaminofluorene ( 2-AAF ) with a two-thirds partial hepatectomy ( PH ) performed after the first week of 2-AAF treatment ( modified Solt-Farber model ) .
	manualset3
161798	9	411941	7	NULL	NULL	0	NULL	partial hepatectomy ( PH )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The question of a possible precursor -- product relationship between oval cells and hepatocytes was examined in rats treated for 2 weeks with 2-acetylaminofluorene ( 2-AAF ) with a two-thirds partial hepatectomy ( PH ) performed after the first week of 2-AAF treatment ( modified Solt-Farber model ) .
	manualset3
161799	10	411941	7	NULL	NULL	0	NULL	first week	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The question of a possible precursor -- product relationship between oval cells and hepatocytes was examined in rats treated for 2 weeks with 2-acetylaminofluorene ( 2-AAF ) with a two-thirds partial hepatectomy ( PH ) performed after the first week of 2-AAF treatment ( modified Solt-Farber model ) .
	manualset3
161800	11	411941	7	NULL	NULL	0	NULL	2-AAF treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The question of a possible precursor -- product relationship between oval cells and hepatocytes was examined in rats treated for 2 weeks with 2-acetylaminofluorene ( 2-AAF ) with a two-thirds partial hepatectomy ( PH ) performed after the first week of 2-AAF treatment ( modified Solt-Farber model ) .
	manualset3
161801	12	411941	7	NULL	NULL	0	NULL	modified Solt-Farber model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The question of a possible precursor -- product relationship between oval cells and hepatocytes was examined in rats treated for 2 weeks with 2-acetylaminofluorene ( 2-AAF ) with a two-thirds partial hepatectomy ( PH ) performed after the first week of 2-AAF treatment ( modified Solt-Farber model ) .
	manualset3
161802	1	411942	7	NULL	NULL	0	NULL	question 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The question of whether Przewalski 's horse is the direct progenitor of domestic horse has been hotly debated .
	manualset3
161803	2	411942	7	NULL	NULL	0	NULL	Przewalski 's horse	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The question of whether Przewalski 's horse is the direct progenitor of domestic horse has been hotly debated .
	manualset3
161804	3	411942	7	NULL	NULL	0	NULL	direct progenitor	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The question of whether Przewalski 's horse is the direct progenitor of domestic horse has been hotly debated .
	manualset3
161805	4	411942	7	NULL	NULL	0	NULL	domestic horse	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The question of whether Przewalski 's horse is the direct progenitor of domestic horse has been hotly debated .
	manualset3
161806	1	411943	7	NULL	NULL	0	NULL	question	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The question remains as to whether positive responders to the 35 % CO ( 2 ) inhalation ( more specifically PD patients ) show a more pronounced HPA axis response .
	manualset3
161807	2	411943	7	NULL	NULL	0	NULL	positive responders 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The question remains as to whether positive responders to the 35 % CO ( 2 ) inhalation ( more specifically PD patients ) show a more pronounced HPA axis response .
	manualset3
161808	3	411943	7	NULL	NULL	0	NULL	 35 % CO ( 2 ) inhalation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The question remains as to whether positive responders to the 35 % CO ( 2 ) inhalation ( more specifically PD patients ) show a more pronounced HPA axis response .
	manualset3
161809	4	411943	7	NULL	NULL	0	NULL	PD patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The question remains as to whether positive responders to the 35 % CO ( 2 ) inhalation ( more specifically PD patients ) show a more pronounced HPA axis response .
	manualset3
161810	5	411943	7	NULL	NULL	0	NULL	HPA axis response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The question remains as to whether positive responders to the 35 % CO ( 2 ) inhalation ( more specifically PD patients ) show a more pronounced HPA axis response .
	manualset3
161811	1	411944	7	NULL	NULL	0	NULL	 question 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The question that remains is not whether IMAC can be active at physiological concentrations of Mg2 + and H + , but what other factors might increase its sensitivity to changes in mitochondrial volume .
	manualset3
161812	2	411944	7	NULL	NULL	0	NULL	IMAC	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The question that remains is not whether IMAC can be active at physiological concentrations of Mg2 + and H + , but what other factors might increase its sensitivity to changes in mitochondrial volume .
	manualset3
161813	3	411944	7	NULL	NULL	0	NULL	physiological concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The question that remains is not whether IMAC can be active at physiological concentrations of Mg2 + and H + , but what other factors might increase its sensitivity to changes in mitochondrial volume .
	manualset3
161814	4	411944	7	NULL	NULL	0	NULL	Mg2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The question that remains is not whether IMAC can be active at physiological concentrations of Mg2 + and H + , but what other factors might increase its sensitivity to changes in mitochondrial volume .
	manualset3
161815	5	411944	7	NULL	NULL	0	NULL	H +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The question that remains is not whether IMAC can be active at physiological concentrations of Mg2 + and H + , but what other factors might increase its sensitivity to changes in mitochondrial volume .
	manualset3
161816	6	411944	7	NULL	NULL	0	NULL	factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The question that remains is not whether IMAC can be active at physiological concentrations of Mg2 + and H + , but what other factors might increase its sensitivity to changes in mitochondrial volume .
	manualset3
161817	7	411944	7	NULL	NULL	0	NULL	sensitivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The question that remains is not whether IMAC can be active at physiological concentrations of Mg2 + and H + , but what other factors might increase its sensitivity to changes in mitochondrial volume .
	manualset3
161818	8	411944	7	NULL	NULL	0	NULL	mitochondrial volume	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The question that remains is not whether IMAC can be active at physiological concentrations of Mg2 + and H + , but what other factors might increase its sensitivity to changes in mitochondrial volume .
	manualset3
161819	1	411945	7	NULL	NULL	0	NULL	questionnaire	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The questionnaire concerned among others : nutrition regularity , consumption frequency , preference levels of different kinds of food products , the knowledge of atherosclerosis prevention rules and the health condition of the respondents as well .
	manualset3
161820	2	411945	7	NULL	NULL	0	NULL	 nutrition regularity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The questionnaire concerned among others : nutrition regularity , consumption frequency , preference levels of different kinds of food products , the knowledge of atherosclerosis prevention rules and the health condition of the respondents as well .
	manualset3
161821	3	411945	7	NULL	NULL	0	NULL	consumption frequency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The questionnaire concerned among others : nutrition regularity , consumption frequency , preference levels of different kinds of food products , the knowledge of atherosclerosis prevention rules and the health condition of the respondents as well .
	manualset3
161822	4	411945	7	NULL	NULL	0	NULL	food products	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The questionnaire concerned among others : nutrition regularity , consumption frequency , preference levels of different kinds of food products , the knowledge of atherosclerosis prevention rules and the health condition of the respondents as well .
	manualset3
161823	5	411945	7	NULL	NULL	0	NULL	knowledge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The questionnaire concerned among others : nutrition regularity , consumption frequency , preference levels of different kinds of food products , the knowledge of atherosclerosis prevention rules and the health condition of the respondents as well .
	manualset3
161824	6	411945	7	NULL	NULL	0	NULL	atherosclerosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The questionnaire concerned among others : nutrition regularity , consumption frequency , preference levels of different kinds of food products , the knowledge of atherosclerosis prevention rules and the health condition of the respondents as well .
	manualset3
161825	7	411945	7	NULL	NULL	NULL	NULL	prevention	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The questionnaire concerned among others : nutrition regularity , consumption frequency , preference levels of different kinds of food products , the knowledge of atherosclerosis prevention rules and the health condition of the respondents as well .
	manualset3
161826	9	411945	7	NULL	NULL	NULL	NULL	health condition	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The questionnaire concerned among others : nutrition regularity , consumption frequency , preference levels of different kinds of food products , the knowledge of atherosclerosis prevention rules and the health condition of the respondents as well .
	manualset3
161827	10	411945	7	NULL	NULL	NULL	NULL	respondents	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The questionnaire concerned among others : nutrition regularity , consumption frequency , preference levels of different kinds of food products , the knowledge of atherosclerosis prevention rules and the health condition of the respondents as well .
	manualset3
161828	8	411945	7	NULL	NULL	NULL	NULL	rules	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The questionnaire concerned among others : nutrition regularity , consumption frequency , preference levels of different kinds of food products , the knowledge of atherosclerosis prevention rules and the health condition of the respondents as well .
	manualset3
161829	1	411946	7	NULL	NULL	0	NULL	radiation levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The radiation levels in the cyclotron and radiochemistry laboratory were observed to be well within prescribed limits with safe work practice .
	manualset3
161830	2	411946	7	NULL	NULL	0	NULL	 cyclotron	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The radiation levels in the cyclotron and radiochemistry laboratory were observed to be well within prescribed limits with safe work practice .
	manualset3
161831	3	411946	7	NULL	NULL	0	NULL	 radiochemistry laboratory	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The radiation levels in the cyclotron and radiochemistry laboratory were observed to be well within prescribed limits with safe work practice .
	manualset3
161832	4	411946	7	NULL	NULL	0	NULL	limits	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The radiation levels in the cyclotron and radiochemistry laboratory were observed to be well within prescribed limits with safe work practice .
	manualset3
161833	5	411946	7	NULL	NULL	0	NULL	safe work practice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The radiation levels in the cyclotron and radiochemistry laboratory were observed to be well within prescribed limits with safe work practice .
	manualset3
161834	1	411947	7	NULL	NULL	0	NULL	radiation sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The radiation sensitivity of leukemic progenitor cells in 12 cases of acute nonlymphocytic leukemia was compared with that of normal myeloid progenitor cells ( colony-forming units in culture ) , using in vitro cloning techniques .
	manualset3
161835	2	411947	7	NULL	NULL	0	NULL	leukemic progenitor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The radiation sensitivity of leukemic progenitor cells in 12 cases of acute nonlymphocytic leukemia was compared with that of normal myeloid progenitor cells ( colony-forming units in culture ) , using in vitro cloning techniques .
	manualset3
161836	3	411947	7	NULL	NULL	0	NULL	12 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The radiation sensitivity of leukemic progenitor cells in 12 cases of acute nonlymphocytic leukemia was compared with that of normal myeloid progenitor cells ( colony-forming units in culture ) , using in vitro cloning techniques .
	manualset3
161837	4	411947	7	NULL	NULL	0	NULL	acute nonlymphocytic leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The radiation sensitivity of leukemic progenitor cells in 12 cases of acute nonlymphocytic leukemia was compared with that of normal myeloid progenitor cells ( colony-forming units in culture ) , using in vitro cloning techniques .
	manualset3
161838	5	411947	7	NULL	NULL	0	NULL	normal myeloid progenitor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The radiation sensitivity of leukemic progenitor cells in 12 cases of acute nonlymphocytic leukemia was compared with that of normal myeloid progenitor cells ( colony-forming units in culture ) , using in vitro cloning techniques .
	manualset3
161839	6	411947	7	NULL	NULL	0	NULL	colony-forming units	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The radiation sensitivity of leukemic progenitor cells in 12 cases of acute nonlymphocytic leukemia was compared with that of normal myeloid progenitor cells ( colony-forming units in culture ) , using in vitro cloning techniques .
	manualset3
161840	7	411947	7	NULL	NULL	0	NULL	culture 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The radiation sensitivity of leukemic progenitor cells in 12 cases of acute nonlymphocytic leukemia was compared with that of normal myeloid progenitor cells ( colony-forming units in culture ) , using in vitro cloning techniques .
	manualset3
161841	8	411947	7	NULL	NULL	0	NULL	in vitro cloning techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The radiation sensitivity of leukemic progenitor cells in 12 cases of acute nonlymphocytic leukemia was compared with that of normal myeloid progenitor cells ( colony-forming units in culture ) , using in vitro cloning techniques .
	manualset3
161842	1	411948	7	NULL	NULL	0	NULL	Aberrant regeneration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Aberrant regeneration of the oculomotor nerve may occur months to years after the occurrence of an oculomotor lesion .
	manualset3
161843	2	411948	7	NULL	NULL	0	NULL	oculomotor nerve	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Aberrant regeneration of the oculomotor nerve may occur months to years after the occurrence of an oculomotor lesion .
	manualset3
161844	3	411948	7	NULL	NULL	0	NULL	months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Aberrant regeneration of the oculomotor nerve may occur months to years after the occurrence of an oculomotor lesion .
	manualset3
161845	4	411948	7	NULL	NULL	0	NULL	years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Aberrant regeneration of the oculomotor nerve may occur months to years after the occurrence of an oculomotor lesion .
	manualset3
161846	5	411948	7	NULL	NULL	0	NULL	occurrence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Aberrant regeneration of the oculomotor nerve may occur months to years after the occurrence of an oculomotor lesion .
	manualset3
161847	6	411948	7	NULL	NULL	0	NULL	oculomotor lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Aberrant regeneration of the oculomotor nerve may occur months to years after the occurrence of an oculomotor lesion .
	manualset3
161848	1	411949	7	NULL	NULL	NULL	NULL	radiological assessment 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The radiological assessment of bladder emptying .
	manualset3
161849	2	411949	7	NULL	NULL	NULL	NULL	bladder emptying	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The radiological assessment of bladder emptying .
	manualset3
161850	1	411950	7	NULL	NULL	0	NULL	radiological magnification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The radiological magnification of an object is illustrated as a ratio of planes .
	manualset3
161851	2	411950	7	NULL	NULL	0	NULL	object	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The radiological magnification of an object is illustrated as a ratio of planes .
	manualset3
161852	3	411950	7	NULL	NULL	0	NULL	ratio of planes	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The radiological magnification of an object is illustrated as a ratio of planes .
	manualset3
161853	1	411951	7	NULL	NULL	0	NULL	radiosensitivity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The radiosensitivity of human neuroblastoma : a cellular and molecular study .
	manualset3
161854	2	411951	7	NULL	NULL	0	NULL	human neuroblastoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The radiosensitivity of human neuroblastoma : a cellular and molecular study .
	manualset3
161855	3	411951	7	NULL	NULL	0	NULL	cellular and molecular study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The radiosensitivity of human neuroblastoma : a cellular and molecular study .
	manualset3
161856	1	411952	7	NULL	NULL	NULL	NULL	 radon level	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The radon level in underground buildings has the lowest value in winter and the highest value in summer .
	manualset3
161857	2	411952	7	NULL	NULL	0	NULL	underground buildings	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The radon level in underground buildings has the lowest value in winter and the highest value in summer .
	manualset3
161858	3	411952	7	NULL	NULL	0	NULL	lowest value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The radon level in underground buildings has the lowest value in winter and the highest value in summer .
	manualset3
161859	4	411952	7	NULL	NULL	NULL	NULL	winter	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The radon level in underground buildings has the lowest value in winter and the highest value in summer .
	manualset3
161860	5	411952	7	NULL	NULL	0	NULL	highest value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The radon level in underground buildings has the lowest value in winter and the highest value in summer .
	manualset3
161861	6	411952	7	NULL	NULL	NULL	NULL	summer	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The radon level in underground buildings has the lowest value in winter and the highest value in summer .
	manualset3
161862	1	411953	7	NULL	NULL	0	NULL	random effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The random effect of sire was included to estimate additive genetic effects , which were assumed to be continuous for IMF , MS , and SC , but a probit threshold link function was fitted for HP .
	manualset3
161863	2	411953	7	NULL	NULL	0	NULL	sire	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The random effect of sire was included to estimate additive genetic effects , which were assumed to be continuous for IMF , MS , and SC , but a probit threshold link function was fitted for HP .
	manualset3
161864	3	411953	7	NULL	NULL	0	NULL	additive genetic effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The random effect of sire was included to estimate additive genetic effects , which were assumed to be continuous for IMF , MS , and SC , but a probit threshold link function was fitted for HP .
	manualset3
161865	4	411953	7	NULL	NULL	NULL	NULL	 IMF	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The random effect of sire was included to estimate additive genetic effects , which were assumed to be continuous for IMF , MS , and SC , but a probit threshold link function was fitted for HP .
	manualset3
161866	5	411953	7	NULL	NULL	0	NULL	MS	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The random effect of sire was included to estimate additive genetic effects , which were assumed to be continuous for IMF , MS , and SC , but a probit threshold link function was fitted for HP .
	manualset3
161867	6	411953	7	NULL	NULL	0	NULL	SC	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The random effect of sire was included to estimate additive genetic effects , which were assumed to be continuous for IMF , MS , and SC , but a probit threshold link function was fitted for HP .
	manualset3
161868	7	411953	7	NULL	NULL	NULL	NULL	probit threshold link function 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The random effect of sire was included to estimate additive genetic effects , which were assumed to be continuous for IMF , MS , and SC , but a probit threshold link function was fitted for HP .
	manualset3
161869	8	411953	7	NULL	NULL	0	NULL	HP 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The random effect of sire was included to estimate additive genetic effects , which were assumed to be continuous for IMF , MS , and SC , but a probit threshold link function was fitted for HP .
	manualset3
161870	1	411954	7	NULL	NULL	0	NULL	 range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The range of serum MEP concentrations were from undetectable level ( & lt ; 0.01 microg/mL ) to 9.73 microg/mL .
	manualset3
161871	2	411954	7	NULL	NULL	0	NULL	serum MEP concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The range of serum MEP concentrations were from undetectable level ( & lt ; 0.01 microg/mL ) to 9.73 microg/mL .
	manualset3
161872	3	411954	7	NULL	NULL	0	NULL	undetectable level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The range of serum MEP concentrations were from undetectable level ( & lt ; 0.01 microg/mL ) to 9.73 microg/mL .
	manualset3
161873	4	411954	7	NULL	NULL	0	NULL	0.01 microg/mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The range of serum MEP concentrations were from undetectable level ( & lt ; 0.01 microg/mL ) to 9.73 microg/mL .
	manualset3
161874	5	411954	7	NULL	NULL	0	NULL	9.73 microg/mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The range of serum MEP concentrations were from undetectable level ( & lt ; 0.01 microg/mL ) to 9.73 microg/mL .
	manualset3
161875	1	411955	7	NULL	NULL	0	NULL	 range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The range of the laterality was rather considerable because the coefficient differed from 1.02 to 3.6 .
	manualset3
161876	2	411955	7	NULL	NULL	0	NULL	laterality	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The range of the laterality was rather considerable because the coefficient differed from 1.02 to 3.6 .
	manualset3
161877	3	411955	7	NULL	NULL	0	NULL	 coefficient	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The range of the laterality was rather considerable because the coefficient differed from 1.02 to 3.6 .
	manualset3
161878	4	411955	7	NULL	NULL	0	NULL	1.02 to 3.6	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The range of the laterality was rather considerable because the coefficient differed from 1.02 to 3.6 .
	manualset3
161879	1	411956	7	NULL	NULL	0	NULL	raphe pallidus ( RPa ) 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The raphe pallidus ( RPa ) and Btzinger complex ( BtC ) represent two important nuclei which project to spinal phrenic motor neurons .
	manualset3
161880	2	411956	7	NULL	NULL	0	NULL	Btzinger complex ( BtC )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The raphe pallidus ( RPa ) and Btzinger complex ( BtC ) represent two important nuclei which project to spinal phrenic motor neurons .
	manualset3
161881	3	411956	7	NULL	NULL	0	NULL	nuclei	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The raphe pallidus ( RPa ) and Btzinger complex ( BtC ) represent two important nuclei which project to spinal phrenic motor neurons .
	manualset3
161882	4	411956	7	NULL	NULL	0	NULL	spinal phrenic motor neurons	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The raphe pallidus ( RPa ) and Btzinger complex ( BtC ) represent two important nuclei which project to spinal phrenic motor neurons .
	manualset3
161883	1	411957	7	NULL	NULL	0	NULL	 workforce	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The rapid aging of the workforce in most developed countries , and the strengthening presence of bridge employment among older employees , has brought about a need for a deeper theoretical and practical understanding of this employment phenomenon .
	manualset3
161884	2	411957	7	NULL	NULL	0	NULL	developed countries	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The rapid aging of the workforce in most developed countries , and the strengthening presence of bridge employment among older employees , has brought about a need for a deeper theoretical and practical understanding of this employment phenomenon .
	manualset3
161885	3	411957	7	NULL	NULL	0	NULL	 employment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The rapid aging of the workforce in most developed countries , and the strengthening presence of bridge employment among older employees , has brought about a need for a deeper theoretical and practical understanding of this employment phenomenon .
	manualset3
161886	4	411957	7	NULL	NULL	0	NULL	older employees	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The rapid aging of the workforce in most developed countries , and the strengthening presence of bridge employment among older employees , has brought about a need for a deeper theoretical and practical understanding of this employment phenomenon .
	manualset3
161887	5	411957	7	NULL	NULL	NULL	NULL	theoretical understanding	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The rapid aging of the workforce in most developed countries , and the strengthening presence of bridge employment among older employees , has brought about a need for a deeper theoretical and practical understanding of this employment phenomenon .
	manualset3
161888	6	411957	7	NULL	NULL	NULL	NULL	practical understanding	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The rapid aging of the workforce in most developed countries , and the strengthening presence of bridge employment among older employees , has brought about a need for a deeper theoretical and practical understanding of this employment phenomenon .
	manualset3
161889	7	411957	7	NULL	NULL	0	NULL	 employment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The rapid aging of the workforce in most developed countries , and the strengthening presence of bridge employment among older employees , has brought about a need for a deeper theoretical and practical understanding of this employment phenomenon .
	manualset3
161890	8	411957	7	NULL	NULL	0	NULL	phenomenon 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The rapid aging of the workforce in most developed countries , and the strengthening presence of bridge employment among older employees , has brought about a need for a deeper theoretical and practical understanding of this employment phenomenon .
	manualset3
161891	9	411957	7	NULL	NULL	0	NULL	rapid aging	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The rapid aging of the workforce in most developed countries , and the strengthening presence of bridge employment among older employees , has brought about a need for a deeper theoretical and practical understanding of this employment phenomenon .
	manualset3
162362	10	411957	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The rapid aging of the workforce in most developed countries , and the strengthening presence of bridge employment among older employees , has brought about a need for a deeper theoretical and practical understanding of this employment phenomenon .
	manualset3
161892	1	411958	7	NULL	NULL	0	NULL	ras-related mouse ypt1 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The ras-related mouse ypt1 protein can functionally replace the YPT1 gene product in yeast .
	manualset3
161893	2	411958	7	NULL	NULL	0	NULL	YPT1 gene product	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The ras-related mouse ypt1 protein can functionally replace the YPT1 gene product in yeast .
	manualset3
161894	3	411958	7	NULL	NULL	0	NULL	yeast	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The ras-related mouse ypt1 protein can functionally replace the YPT1 gene product in yeast .
	manualset3
161895	1	411959	7	NULL	NULL	0	NULL	rat L5/6 facet joint 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The rat L5/6 facet joint , from which low back pain can originate , is multisegmentally innervated from the L1 to L5 dorsal root ganglia ( DRG ) .
	manualset3
161896	2	411959	7	NULL	NULL	0	NULL	low back pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The rat L5/6 facet joint , from which low back pain can originate , is multisegmentally innervated from the L1 to L5 dorsal root ganglia ( DRG ) .
	manualset3
161897	3	411959	7	NULL	NULL	0	NULL	L1 to L5 dorsal root ganglia ( DRG )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The rat L5/6 facet joint , from which low back pain can originate , is multisegmentally innervated from the L1 to L5 dorsal root ganglia ( DRG ) .
	manualset3
161898	1	411960	7	NULL	NULL	0	NULL	rat hypothalamus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The rat hypothalamus in vitro preparation was used to investigate the effect of bilateral adrenalectomy , with and without replacement therapy , on the release of corticotrophin-releasing factor ( CRF ) .
	manualset3
161899	2	411960	7	NULL	NULL	0	NULL	in vitro preparation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rat hypothalamus in vitro preparation was used to investigate the effect of bilateral adrenalectomy , with and without replacement therapy , on the release of corticotrophin-releasing factor ( CRF ) .
	manualset3
161900	3	411960	7	NULL	NULL	0	NULL	effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The rat hypothalamus in vitro preparation was used to investigate the effect of bilateral adrenalectomy , with and without replacement therapy , on the release of corticotrophin-releasing factor ( CRF ) .
	manualset3
161901	4	411960	7	NULL	NULL	0	NULL	bilateral adrenalectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The rat hypothalamus in vitro preparation was used to investigate the effect of bilateral adrenalectomy , with and without replacement therapy , on the release of corticotrophin-releasing factor ( CRF ) .
	manualset3
161902	5	411960	7	NULL	NULL	0	NULL	replacement therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The rat hypothalamus in vitro preparation was used to investigate the effect of bilateral adrenalectomy , with and without replacement therapy , on the release of corticotrophin-releasing factor ( CRF ) .
	manualset3
161903	6	411960	7	NULL	NULL	0	NULL	release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The rat hypothalamus in vitro preparation was used to investigate the effect of bilateral adrenalectomy , with and without replacement therapy , on the release of corticotrophin-releasing factor ( CRF ) .
	manualset3
161904	7	411960	7	NULL	NULL	0	NULL	corticotrophin-releasing factor ( CRF )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The rat hypothalamus in vitro preparation was used to investigate the effect of bilateral adrenalectomy , with and without replacement therapy , on the release of corticotrophin-releasing factor ( CRF ) .
	manualset3
161905	1	411961	7	NULL	NULL	0	NULL	rat thalamic nucleus submedius 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The rat thalamic nucleus submedius responds to noxious pressure stimuli in the colon .
	manualset3
161906	2	411961	7	NULL	NULL	0	NULL	noxious pressure stimuli	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The rat thalamic nucleus submedius responds to noxious pressure stimuli in the colon .
	manualset3
161907	3	411961	7	NULL	NULL	0	NULL	colon	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The rat thalamic nucleus submedius responds to noxious pressure stimuli in the colon .
	manualset3
161908	1	411962	7	NULL	NULL	NULL	NULL	rate-limiting step	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The rate-limiting step during the refolding of S54G/P55N ribonuclease T1 is determined by the slow trans -- ) cis prolyl isomerisation of Pro39 .
	manualset3
161909	2	411962	7	NULL	NULL	0	NULL	 refolding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate-limiting step during the refolding of S54G/P55N ribonuclease T1 is determined by the slow trans -- ) cis prolyl isomerisation of Pro39 .
	manualset3
161910	3	411962	7	NULL	NULL	0	NULL	S54G/P55N ribonuclease T1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate-limiting step during the refolding of S54G/P55N ribonuclease T1 is determined by the slow trans -- ) cis prolyl isomerisation of Pro39 .
	manualset3
161911	4	411962	7	NULL	NULL	0	NULL	slow trans -- ) cis prolyl isomerisation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate-limiting step during the refolding of S54G/P55N ribonuclease T1 is determined by the slow trans -- ) cis prolyl isomerisation of Pro39 .
	manualset3
161912	5	411962	7	NULL	NULL	0	NULL	Pro39	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate-limiting step during the refolding of S54G/P55N ribonuclease T1 is determined by the slow trans -- ) cis prolyl isomerisation of Pro39 .
	manualset3
161913	1	411963	7	NULL	NULL	0	NULL	rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate and magnitude of contraction with 80 mm KCl ( depolarizing ) was decreased in lactate-PSS ( P = 0.001 ) .
	manualset3
161914	2	411963	7	NULL	NULL	0	NULL	 magnitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate and magnitude of contraction with 80 mm KCl ( depolarizing ) was decreased in lactate-PSS ( P = 0.001 ) .
	manualset3
161915	3	411963	7	NULL	NULL	0	NULL	contraction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate and magnitude of contraction with 80 mm KCl ( depolarizing ) was decreased in lactate-PSS ( P = 0.001 ) .
	manualset3
161916	4	411963	7	NULL	NULL	0	NULL	80 mm KCl	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate and magnitude of contraction with 80 mm KCl ( depolarizing ) was decreased in lactate-PSS ( P = 0.001 ) .
	manualset3
161918	6	411963	7	NULL	NULL	0	NULL	lactate-PSS	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate and magnitude of contraction with 80 mm KCl ( depolarizing ) was decreased in lactate-PSS ( P = 0.001 ) .
	manualset3
161919	7	411963	7	NULL	NULL	0	NULL	P = 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate and magnitude of contraction with 80 mm KCl ( depolarizing ) was decreased in lactate-PSS ( P = 0.001 ) .
	manualset3
161920	1	411964	7	NULL	NULL	0	NULL	rate constant	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate constant of bacteria in the presence of the drugs decreased with increasing concentrations of the drugs .
	manualset3
161921	2	411964	7	NULL	NULL	0	NULL	bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate constant of bacteria in the presence of the drugs decreased with increasing concentrations of the drugs .
	manualset3
161922	3	411964	7	NULL	NULL	0	NULL	drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate constant of bacteria in the presence of the drugs decreased with increasing concentrations of the drugs .
	manualset3
161923	4	411964	7	NULL	NULL	0	NULL	increasing concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate constant of bacteria in the presence of the drugs decreased with increasing concentrations of the drugs .
	manualset3
161924	5	411964	7	NULL	NULL	0	NULL	drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate constant of bacteria in the presence of the drugs decreased with increasing concentrations of the drugs .
	manualset3
169468	6	411964	7	NULL	NULL	0	NULL	presence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate constant of bacteria in the presence of the drugs decreased with increasing concentrations of the drugs .
	manualset3
161925	1	411965	7	NULL	NULL	0	NULL	thymic lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Ability of thymic lymphocytes to alter CFU kinetics in radiation chimeras .
	manualset3
161926	2	411965	7	NULL	NULL	0	NULL	CFU kinetics	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ability of thymic lymphocytes to alter CFU kinetics in radiation chimeras .
	manualset3
161927	3	411965	7	NULL	NULL	0	NULL	radiation chimeras	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Ability of thymic lymphocytes to alter CFU kinetics in radiation chimeras .
	manualset3
161928	1	411966	7	NULL	NULL	0	NULL	rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate increases linearly with either stroke ( S ) or frequency ( n ) above a certain value ( S = 5 mm or n = 10Hz ) .
	manualset3
161929	2	411966	7	NULL	NULL	0	NULL	 stroke ( S )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate increases linearly with either stroke ( S ) or frequency ( n ) above a certain value ( S = 5 mm or n = 10Hz ) .
	manualset3
161930	3	411966	7	NULL	NULL	0	NULL	frequency ( n )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate increases linearly with either stroke ( S ) or frequency ( n ) above a certain value ( S = 5 mm or n = 10Hz ) .
	manualset3
161931	4	411966	7	NULL	NULL	0	NULL	value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate increases linearly with either stroke ( S ) or frequency ( n ) above a certain value ( S = 5 mm or n = 10Hz ) .
	manualset3
161932	5	411966	7	NULL	NULL	0	NULL	S = 5 mm or n = 10Hz	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate increases linearly with either stroke ( S ) or frequency ( n ) above a certain value ( S = 5 mm or n = 10Hz ) .
	manualset3
161933	1	411967	7	NULL	NULL	0	NULL	rate 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of ESBL - and qnr-positive isolates was 7 % and 14 % , respectively .
	manualset3
161934	2	411967	7	NULL	NULL	0	NULL	ESBL - positive isolates	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of ESBL - and qnr-positive isolates was 7 % and 14 % , respectively .
	manualset3
161935	3	411967	7	NULL	NULL	0	NULL	qnr-positive isolates	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of ESBL - and qnr-positive isolates was 7 % and 14 % , respectively .
	manualset3
161936	4	411967	7	NULL	NULL	0	NULL	7 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of ESBL - and qnr-positive isolates was 7 % and 14 % , respectively .
	manualset3
161937	5	411967	7	NULL	NULL	0	NULL	14 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of ESBL - and qnr-positive isolates was 7 % and 14 % , respectively .
	manualset3
161938	1	411968	7	NULL	NULL	0	NULL	 rate 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of albumin synthesis is inversely proportional to the serum concentration of one potential acute phase protein ( alpha2 macroglobulin ) , and albumin concentration is inversely proportional to that of either C-reactive protein or serum amyloid A in both HD and PD patients .
	manualset3
161939	2	411968	7	NULL	NULL	0	NULL	albumin synthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of albumin synthesis is inversely proportional to the serum concentration of one potential acute phase protein ( alpha2 macroglobulin ) , and albumin concentration is inversely proportional to that of either C-reactive protein or serum amyloid A in both HD and PD patients .
	manualset3
161940	3	411968	7	NULL	NULL	0	NULL	serum concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of albumin synthesis is inversely proportional to the serum concentration of one potential acute phase protein ( alpha2 macroglobulin ) , and albumin concentration is inversely proportional to that of either C-reactive protein or serum amyloid A in both HD and PD patients .
	manualset3
161941	4	411968	7	NULL	NULL	0	NULL	one potential acute phase protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of albumin synthesis is inversely proportional to the serum concentration of one potential acute phase protein ( alpha2 macroglobulin ) , and albumin concentration is inversely proportional to that of either C-reactive protein or serum amyloid A in both HD and PD patients .
	manualset3
161942	5	411968	7	NULL	NULL	0	NULL	alpha2 macroglobulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of albumin synthesis is inversely proportional to the serum concentration of one potential acute phase protein ( alpha2 macroglobulin ) , and albumin concentration is inversely proportional to that of either C-reactive protein or serum amyloid A in both HD and PD patients .
	manualset3
161943	6	411968	7	NULL	NULL	0	NULL	albumin concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of albumin synthesis is inversely proportional to the serum concentration of one potential acute phase protein ( alpha2 macroglobulin ) , and albumin concentration is inversely proportional to that of either C-reactive protein or serum amyloid A in both HD and PD patients .
	manualset3
161944	7	411968	7	NULL	NULL	0	NULL	C-reactive protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of albumin synthesis is inversely proportional to the serum concentration of one potential acute phase protein ( alpha2 macroglobulin ) , and albumin concentration is inversely proportional to that of either C-reactive protein or serum amyloid A in both HD and PD patients .
	manualset3
161945	8	411968	7	NULL	NULL	0	NULL	serum amyloid A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of albumin synthesis is inversely proportional to the serum concentration of one potential acute phase protein ( alpha2 macroglobulin ) , and albumin concentration is inversely proportional to that of either C-reactive protein or serum amyloid A in both HD and PD patients .
	manualset3
161946	9	411968	7	NULL	NULL	0	NULL	HD patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of albumin synthesis is inversely proportional to the serum concentration of one potential acute phase protein ( alpha2 macroglobulin ) , and albumin concentration is inversely proportional to that of either C-reactive protein or serum amyloid A in both HD and PD patients .
	manualset3
161947	10	411968	7	NULL	NULL	0	NULL	PD patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of albumin synthesis is inversely proportional to the serum concentration of one potential acute phase protein ( alpha2 macroglobulin ) , and albumin concentration is inversely proportional to that of either C-reactive protein or serum amyloid A in both HD and PD patients .
	manualset3
161948	1	411969	7	NULL	NULL	0	NULL	 rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of attachment of Fasciola hepatica miracidia to various species of lymnaeid .
	manualset3
161949	2	411969	7	NULL	NULL	0	NULL	attachment	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of attachment of Fasciola hepatica miracidia to various species of lymnaeid .
	manualset3
161950	3	411969	7	NULL	NULL	0	NULL	Fasciola hepatica miracidia	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of attachment of Fasciola hepatica miracidia to various species of lymnaeid .
	manualset3
161951	4	411969	7	NULL	NULL	0	NULL	species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of attachment of Fasciola hepatica miracidia to various species of lymnaeid .
	manualset3
161952	5	411969	7	NULL	NULL	0	NULL	 lymnaeid	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of attachment of Fasciola hepatica miracidia to various species of lymnaeid .
	manualset3
161953	1	411970	7	NULL	NULL	0	NULL	rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of decay was slower in cells from diabetic animals compared with controls .
	manualset3
161954	2	411970	7	NULL	NULL	0	NULL	decay 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of decay was slower in cells from diabetic animals compared with controls .
	manualset3
161955	3	411970	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of decay was slower in cells from diabetic animals compared with controls .
	manualset3
161956	4	411970	7	NULL	NULL	0	NULL	diabetic animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of decay was slower in cells from diabetic animals compared with controls .
	manualset3
161957	5	411970	7	NULL	NULL	0	NULL	controls 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of decay was slower in cells from diabetic animals compared with controls .
	manualset3
161958	1	411971	7	NULL	NULL	0	NULL	 rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of neurologic progression in the four patients with childhood ALD did not differ from that of 167 untreated patients with childhood ALD surveyed previously .
	manualset3
161959	2	411971	7	NULL	NULL	0	NULL	neurologic progression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of neurologic progression in the four patients with childhood ALD did not differ from that of 167 untreated patients with childhood ALD surveyed previously .
	manualset3
161960	3	411971	7	NULL	NULL	0	NULL	four patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of neurologic progression in the four patients with childhood ALD did not differ from that of 167 untreated patients with childhood ALD surveyed previously .
	manualset3
161961	4	411971	7	NULL	NULL	0	NULL	childhood ALD	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of neurologic progression in the four patients with childhood ALD did not differ from that of 167 untreated patients with childhood ALD surveyed previously .
	manualset3
161962	5	411971	7	NULL	NULL	NULL	NULL	167 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The rate of neurologic progression in the four patients with childhood ALD did not differ from that of 167 untreated patients with childhood ALD surveyed previously .
	manualset3
161963	7	411971	7	NULL	NULL	NULL	NULL	childhood ALD	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The rate of neurologic progression in the four patients with childhood ALD did not differ from that of 167 untreated patients with childhood ALD surveyed previously .
	manualset3
161964	6	411971	7	NULL	NULL	0	NULL	untreated patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of neurologic progression in the four patients with childhood ALD did not differ from that of 167 untreated patients with childhood ALD surveyed previously .
	manualset3
161965	1	411972	7	NULL	NULL	0	NULL	rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of plasmin truncation is similar between the extensively glycosylated COS7-expressed receptor and the nonglycosylated yeast-produced receptor .
	manualset3
161966	2	411972	7	NULL	NULL	0	NULL	plasmin truncation	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of plasmin truncation is similar between the extensively glycosylated COS7-expressed receptor and the nonglycosylated yeast-produced receptor .
	manualset3
161967	3	411972	7	NULL	NULL	0	NULL	glycosylated COS7-expressed receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of plasmin truncation is similar between the extensively glycosylated COS7-expressed receptor and the nonglycosylated yeast-produced receptor .
	manualset3
161968	4	411972	7	NULL	NULL	0	NULL	nonglycosylated yeast-produced receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of plasmin truncation is similar between the extensively glycosylated COS7-expressed receptor and the nonglycosylated yeast-produced receptor .
	manualset3
161969	1	411973	7	NULL	NULL	0	NULL	rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of primary S. marcescens nosocomial bacteremia during the pre-epidemic period ( January-September 1985 ) was 6.25 per cent ; and for the post-epidemic period compared with the epidemic were significantly different ( p & lt ; 0.0001 ) .
	manualset3
161970	2	411973	7	NULL	NULL	0	NULL	 primary S. marcescens nosocomial bacteremia	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of primary S. marcescens nosocomial bacteremia during the pre-epidemic period ( January-September 1985 ) was 6.25 per cent ; and for the post-epidemic period compared with the epidemic were significantly different ( p & lt ; 0.0001 ) .
	manualset3
161971	3	411973	7	NULL	NULL	0	NULL	pre-epidemic period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of primary S. marcescens nosocomial bacteremia during the pre-epidemic period ( January-September 1985 ) was 6.25 per cent ; and for the post-epidemic period compared with the epidemic were significantly different ( p & lt ; 0.0001 ) .
	manualset3
161972	4	411973	7	NULL	NULL	0	NULL	January-September 1985	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of primary S. marcescens nosocomial bacteremia during the pre-epidemic period ( January-September 1985 ) was 6.25 per cent ; and for the post-epidemic period compared with the epidemic were significantly different ( p & lt ; 0.0001 ) .
	manualset3
161973	5	411973	7	NULL	NULL	0	NULL	 6.25 per cent	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of primary S. marcescens nosocomial bacteremia during the pre-epidemic period ( January-September 1985 ) was 6.25 per cent ; and for the post-epidemic period compared with the epidemic were significantly different ( p & lt ; 0.0001 ) .
	manualset3
161974	6	411973	7	NULL	NULL	0	NULL	post-epidemic period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of primary S. marcescens nosocomial bacteremia during the pre-epidemic period ( January-September 1985 ) was 6.25 per cent ; and for the post-epidemic period compared with the epidemic were significantly different ( p & lt ; 0.0001 ) .
	manualset3
161975	7	411973	7	NULL	NULL	0	NULL	epidemic	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of primary S. marcescens nosocomial bacteremia during the pre-epidemic period ( January-September 1985 ) was 6.25 per cent ; and for the post-epidemic period compared with the epidemic were significantly different ( p & lt ; 0.0001 ) .
	manualset3
161976	8	411973	7	NULL	NULL	0	NULL	p & lt ; 0.0001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of primary S. marcescens nosocomial bacteremia during the pre-epidemic period ( January-September 1985 ) was 6.25 per cent ; and for the post-epidemic period compared with the epidemic were significantly different ( p & lt ; 0.0001 ) .
	manualset3
161977	1	411974	7	NULL	NULL	0	NULL	rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of publications was decreased during World Wars I and II and the years following the Trianon treaty .
	manualset3
161978	2	411974	7	NULL	NULL	0	NULL	publications	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of publications was decreased during World Wars I and II and the years following the Trianon treaty .
	manualset3
161979	3	411974	7	NULL	NULL	0	NULL	World Wars I	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of publications was decreased during World Wars I and II and the years following the Trianon treaty .
	manualset3
161980	4	411974	7	NULL	NULL	0	NULL	World Wars II	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of publications was decreased during World Wars I and II and the years following the Trianon treaty .
	manualset3
161981	5	411974	7	NULL	NULL	0	NULL	years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of publications was decreased during World Wars I and II and the years following the Trianon treaty .
	manualset3
161982	6	411974	7	NULL	NULL	0	NULL	Trianon treaty	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of publications was decreased during World Wars I and II and the years following the Trianon treaty .
	manualset3
161983	1	411975	7	NULL	NULL	0	NULL	Ablation therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ablation therapy for the relief of Mnire 's disease .
	manualset3
161984	2	411975	7	NULL	NULL	0	NULL	 relief	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ablation therapy for the relief of Mnire 's disease .
	manualset3
161985	3	411975	7	NULL	NULL	NULL	NULL	Mnire 's disease 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ablation therapy for the relief of Mnire 's disease .
	manualset3
161986	1	411976	7	NULL	NULL	0	NULL	rate 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of release of these TCA cycle constituents was linear with time for at least 48 h regardless of the cell type .
	manualset3
161987	2	411976	7	NULL	NULL	0	NULL	release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of release of these TCA cycle constituents was linear with time for at least 48 h regardless of the cell type .
	manualset3
161988	3	411976	7	NULL	NULL	0	NULL	TCA cycle constituents	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of release of these TCA cycle constituents was linear with time for at least 48 h regardless of the cell type .
	manualset3
161989	4	411976	7	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of release of these TCA cycle constituents was linear with time for at least 48 h regardless of the cell type .
	manualset3
161990	5	411976	7	NULL	NULL	0	NULL	48 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of release of these TCA cycle constituents was linear with time for at least 48 h regardless of the cell type .
	manualset3
161991	6	411976	7	NULL	NULL	0	NULL	cell type	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of release of these TCA cycle constituents was linear with time for at least 48 h regardless of the cell type .
	manualset3
161992	1	411977	7	NULL	NULL	0	NULL	rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rates of admission to hospital increased very little .
	manualset3
161993	2	411977	7	NULL	NULL	0	NULL	admission	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The rates of admission to hospital increased very little .
	manualset3
161994	3	411977	7	NULL	NULL	0	NULL	 hospital	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The rates of admission to hospital increased very little .
	manualset3
161995	1	411978	7	NULL	NULL	0	NULL	rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rates of nitric oxide scavenging by non-mutated and mutated Hb were similar .
	manualset3
161996	2	411978	7	NULL	NULL	0	NULL	nitric oxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The rates of nitric oxide scavenging by non-mutated and mutated Hb were similar .
	manualset3
161997	3	411978	7	NULL	NULL	0	NULL	non-mutated Hb	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The rates of nitric oxide scavenging by non-mutated and mutated Hb were similar .
	manualset3
161998	4	411978	7	NULL	NULL	0	NULL	mutated Hb	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The rates of nitric oxide scavenging by non-mutated and mutated Hb were similar .
	manualset3
161999	1	411979	7	NULL	NULL	0	NULL	 ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of Abeta42 to Abeta40 ( Abeta42/Abeta40 ) secreted by these cells , however , was significantly higher than that secreted by cells expressing wt PS1 , which corroborated findings from a previous report .
	manualset3
162000	2	411979	7	NULL	NULL	NULL	NULL	Abeta42 to Abeta40	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ratio of Abeta42 to Abeta40 ( Abeta42/Abeta40 ) secreted by these cells , however , was significantly higher than that secreted by cells expressing wt PS1 , which corroborated findings from a previous report .
	manualset3
162001	3	411979	7	NULL	NULL	NULL	NULL	( Abeta42/Abeta40 )	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ratio of Abeta42 to Abeta40 ( Abeta42/Abeta40 ) secreted by these cells , however , was significantly higher than that secreted by cells expressing wt PS1 , which corroborated findings from a previous report .
	manualset3
162002	4	411979	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of Abeta42 to Abeta40 ( Abeta42/Abeta40 ) secreted by these cells , however , was significantly higher than that secreted by cells expressing wt PS1 , which corroborated findings from a previous report .
	manualset3
162003	5	411979	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of Abeta42 to Abeta40 ( Abeta42/Abeta40 ) secreted by these cells , however , was significantly higher than that secreted by cells expressing wt PS1 , which corroborated findings from a previous report .
	manualset3
162004	6	411979	7	NULL	NULL	0	NULL	wt PS1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of Abeta42 to Abeta40 ( Abeta42/Abeta40 ) secreted by these cells , however , was significantly higher than that secreted by cells expressing wt PS1 , which corroborated findings from a previous report .
	manualset3
162005	7	411979	7	NULL	NULL	0	NULL	findings 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of Abeta42 to Abeta40 ( Abeta42/Abeta40 ) secreted by these cells , however , was significantly higher than that secreted by cells expressing wt PS1 , which corroborated findings from a previous report .
	manualset3
162006	8	411979	7	NULL	NULL	0	NULL	 report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of Abeta42 to Abeta40 ( Abeta42/Abeta40 ) secreted by these cells , however , was significantly higher than that secreted by cells expressing wt PS1 , which corroborated findings from a previous report .
	manualset3
162007	1	411980	7	NULL	NULL	0	NULL	ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of collagen I/III subtype protein distribution was not significantly different in the non-dilated and angioplastied groups ( 4.88 + / - 1.00 v 4.70 + / - 0.82 , respectively ) .
	manualset3
162008	2	411980	7	NULL	NULL	0	NULL	collagen I/III subtype protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of collagen I/III subtype protein distribution was not significantly different in the non-dilated and angioplastied groups ( 4.88 + / - 1.00 v 4.70 + / - 0.82 , respectively ) .
	manualset3
162009	3	411980	7	NULL	NULL	NULL	NULL	distribution	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ratio of collagen I/III subtype protein distribution was not significantly different in the non-dilated and angioplastied groups ( 4.88 + / - 1.00 v 4.70 + / - 0.82 , respectively ) .
	manualset3
162010	4	411980	7	NULL	NULL	0	NULL	non-dilated groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of collagen I/III subtype protein distribution was not significantly different in the non-dilated and angioplastied groups ( 4.88 + / - 1.00 v 4.70 + / - 0.82 , respectively ) .
	manualset3
162011	5	411980	7	NULL	NULL	0	NULL	angioplastied groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of collagen I/III subtype protein distribution was not significantly different in the non-dilated and angioplastied groups ( 4.88 + / - 1.00 v 4.70 + / - 0.82 , respectively ) .
	manualset3
162012	6	411980	7	NULL	NULL	0	NULL	4.88 + / - 1.00	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of collagen I/III subtype protein distribution was not significantly different in the non-dilated and angioplastied groups ( 4.88 + / - 1.00 v 4.70 + / - 0.82 , respectively ) .
	manualset3
162013	7	411980	7	NULL	NULL	0	NULL	4.70 + / - 0.82	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of collagen I/III subtype protein distribution was not significantly different in the non-dilated and angioplastied groups ( 4.88 + / - 1.00 v 4.70 + / - 0.82 , respectively ) .
	manualset3
162014	1	411981	7	NULL	NULL	0	NULL	ratio 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of deoxyglucose-6-phosphate to deoxyglucose was 60 : 40 and the compounds were eliminated from the inner ear with a half life of approximately 60 min .
	manualset3
162015	2	411981	7	NULL	NULL	0	NULL	deoxyglucose-6-phosphate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of deoxyglucose-6-phosphate to deoxyglucose was 60 : 40 and the compounds were eliminated from the inner ear with a half life of approximately 60 min .
	manualset3
162016	3	411981	7	NULL	NULL	0	NULL	 deoxyglucose	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of deoxyglucose-6-phosphate to deoxyglucose was 60 : 40 and the compounds were eliminated from the inner ear with a half life of approximately 60 min .
	manualset3
162017	4	411981	7	NULL	NULL	0	NULL	60 : 40	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of deoxyglucose-6-phosphate to deoxyglucose was 60 : 40 and the compounds were eliminated from the inner ear with a half life of approximately 60 min .
	manualset3
162018	5	411981	7	NULL	NULL	0	NULL	compounds	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of deoxyglucose-6-phosphate to deoxyglucose was 60 : 40 and the compounds were eliminated from the inner ear with a half life of approximately 60 min .
	manualset3
162019	6	411981	7	NULL	NULL	NULL	NULL	 inner ear	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ratio of deoxyglucose-6-phosphate to deoxyglucose was 60 : 40 and the compounds were eliminated from the inner ear with a half life of approximately 60 min .
	manualset3
162020	7	411981	7	NULL	NULL	0	NULL	half life	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of deoxyglucose-6-phosphate to deoxyglucose was 60 : 40 and the compounds were eliminated from the inner ear with a half life of approximately 60 min .
	manualset3
162021	8	411981	7	NULL	NULL	0	NULL	 60 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of deoxyglucose-6-phosphate to deoxyglucose was 60 : 40 and the compounds were eliminated from the inner ear with a half life of approximately 60 min .
	manualset3
162022	1	411982	7	NULL	NULL	0	NULL	 ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of myocardial hypertrophy and the prevalence of valvular regurgitation were investigated .
	manualset3
162023	2	411982	7	NULL	NULL	0	NULL	myocardial hypertrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of myocardial hypertrophy and the prevalence of valvular regurgitation were investigated .
	manualset3
162024	3	411982	7	NULL	NULL	0	NULL	prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of myocardial hypertrophy and the prevalence of valvular regurgitation were investigated .
	manualset3
162025	4	411982	7	NULL	NULL	0	NULL	valvular regurgitation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of myocardial hypertrophy and the prevalence of valvular regurgitation were investigated .
	manualset3
162026	1	411983	7	NULL	NULL	0	NULL	ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of n-6 / n-3 polyunsaturated fatty acid is considered to be beneficial around three or four .
	manualset3
162027	2	411983	7	NULL	NULL	0	NULL	n-6 / n-3 polyunsaturated fatty acid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of n-6 / n-3 polyunsaturated fatty acid is considered to be beneficial around three or four .
	manualset3
162028	3	411983	7	NULL	NULL	0	NULL	three	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of n-6 / n-3 polyunsaturated fatty acid is considered to be beneficial around three or four .
	manualset3
162029	4	411983	7	NULL	NULL	0	NULL	four	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of n-6 / n-3 polyunsaturated fatty acid is considered to be beneficial around three or four .
	manualset3
162030	1	411984	7	NULL	NULL	0	NULL	 ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of organic mass ( OM ) to organic carbon ( OC ) in PM ( 2.5 ) aerosols at US national parks in the IMPROVE network was estimated experimentally from solvent extraction of sample filters and from the difference between PM ( 2.5 ) mass and chemical constituents other than OC ( mass balance ) in IMPROVE samples from 1988 to 2003 .
	manualset3
162031	2	411984	7	NULL	NULL	0	NULL	organic mass ( OM )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of organic mass ( OM ) to organic carbon ( OC ) in PM ( 2.5 ) aerosols at US national parks in the IMPROVE network was estimated experimentally from solvent extraction of sample filters and from the difference between PM ( 2.5 ) mass and chemical constituents other than OC ( mass balance ) in IMPROVE samples from 1988 to 2003 .
	manualset3
162032	3	411984	7	NULL	NULL	0	NULL	organic carbon ( OC )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of organic mass ( OM ) to organic carbon ( OC ) in PM ( 2.5 ) aerosols at US national parks in the IMPROVE network was estimated experimentally from solvent extraction of sample filters and from the difference between PM ( 2.5 ) mass and chemical constituents other than OC ( mass balance ) in IMPROVE samples from 1988 to 2003 .
	manualset3
162033	4	411984	7	NULL	NULL	0	NULL	PM ( 2.5 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of organic mass ( OM ) to organic carbon ( OC ) in PM ( 2.5 ) aerosols at US national parks in the IMPROVE network was estimated experimentally from solvent extraction of sample filters and from the difference between PM ( 2.5 ) mass and chemical constituents other than OC ( mass balance ) in IMPROVE samples from 1988 to 2003 .
	manualset3
162034	5	411984	7	NULL	NULL	0	NULL	aerosols	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of organic mass ( OM ) to organic carbon ( OC ) in PM ( 2.5 ) aerosols at US national parks in the IMPROVE network was estimated experimentally from solvent extraction of sample filters and from the difference between PM ( 2.5 ) mass and chemical constituents other than OC ( mass balance ) in IMPROVE samples from 1988 to 2003 .
	manualset3
162035	6	411984	7	NULL	NULL	NULL	NULL	US national parks	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ratio of organic mass ( OM ) to organic carbon ( OC ) in PM ( 2.5 ) aerosols at US national parks in the IMPROVE network was estimated experimentally from solvent extraction of sample filters and from the difference between PM ( 2.5 ) mass and chemical constituents other than OC ( mass balance ) in IMPROVE samples from 1988 to 2003 .
	manualset3
162036	7	411984	7	NULL	NULL	0	NULL	IMPROVE network	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of organic mass ( OM ) to organic carbon ( OC ) in PM ( 2.5 ) aerosols at US national parks in the IMPROVE network was estimated experimentally from solvent extraction of sample filters and from the difference between PM ( 2.5 ) mass and chemical constituents other than OC ( mass balance ) in IMPROVE samples from 1988 to 2003 .
	manualset3
162037	8	411984	7	NULL	NULL	0	NULL	solvent extraction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of organic mass ( OM ) to organic carbon ( OC ) in PM ( 2.5 ) aerosols at US national parks in the IMPROVE network was estimated experimentally from solvent extraction of sample filters and from the difference between PM ( 2.5 ) mass and chemical constituents other than OC ( mass balance ) in IMPROVE samples from 1988 to 2003 .
	manualset3
162038	9	411984	7	NULL	NULL	NULL	NULL	sample filters 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ratio of organic mass ( OM ) to organic carbon ( OC ) in PM ( 2.5 ) aerosols at US national parks in the IMPROVE network was estimated experimentally from solvent extraction of sample filters and from the difference between PM ( 2.5 ) mass and chemical constituents other than OC ( mass balance ) in IMPROVE samples from 1988 to 2003 .
	manualset3
162039	10	411984	7	NULL	NULL	NULL	NULL	PM ( 2.5 )	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ratio of organic mass ( OM ) to organic carbon ( OC ) in PM ( 2.5 ) aerosols at US national parks in the IMPROVE network was estimated experimentally from solvent extraction of sample filters and from the difference between PM ( 2.5 ) mass and chemical constituents other than OC ( mass balance ) in IMPROVE samples from 1988 to 2003 .
	manualset3
162040	11	411984	7	NULL	NULL	0	NULL	chemical constituents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of organic mass ( OM ) to organic carbon ( OC ) in PM ( 2.5 ) aerosols at US national parks in the IMPROVE network was estimated experimentally from solvent extraction of sample filters and from the difference between PM ( 2.5 ) mass and chemical constituents other than OC ( mass balance ) in IMPROVE samples from 1988 to 2003 .
	manualset3
162041	12	411984	7	NULL	NULL	0	NULL	OC ( mass balance )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of organic mass ( OM ) to organic carbon ( OC ) in PM ( 2.5 ) aerosols at US national parks in the IMPROVE network was estimated experimentally from solvent extraction of sample filters and from the difference between PM ( 2.5 ) mass and chemical constituents other than OC ( mass balance ) in IMPROVE samples from 1988 to 2003 .
	manualset3
162042	13	411984	7	NULL	NULL	0	NULL	IMPROVE samples	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of organic mass ( OM ) to organic carbon ( OC ) in PM ( 2.5 ) aerosols at US national parks in the IMPROVE network was estimated experimentally from solvent extraction of sample filters and from the difference between PM ( 2.5 ) mass and chemical constituents other than OC ( mass balance ) in IMPROVE samples from 1988 to 2003 .
	manualset3
162043	14	411984	7	NULL	NULL	0	NULL	1988 to 2003	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of organic mass ( OM ) to organic carbon ( OC ) in PM ( 2.5 ) aerosols at US national parks in the IMPROVE network was estimated experimentally from solvent extraction of sample filters and from the difference between PM ( 2.5 ) mass and chemical constituents other than OC ( mass balance ) in IMPROVE samples from 1988 to 2003 .
	manualset3
162509	15	411984	7	NULL	NULL	0	NULL	 mass constituent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of organic mass ( OM ) to organic carbon ( OC ) in PM ( 2.5 ) aerosols at US national parks in the IMPROVE network was estimated experimentally from solvent extraction of sample filters and from the difference between PM ( 2.5 ) mass and chemical constituents other than OC ( mass balance ) in IMPROVE samples from 1988 to 2003 .
	manualset3
162901	16	411984	7	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of organic mass ( OM ) to organic carbon ( OC ) in PM ( 2.5 ) aerosols at US national parks in the IMPROVE network was estimated experimentally from solvent extraction of sample filters and from the difference between PM ( 2.5 ) mass and chemical constituents other than OC ( mass balance ) in IMPROVE samples from 1988 to 2003 .
	manualset3
162044	1	411985	7	NULL	NULL	0	NULL	ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of toxic to lethal doses was 0.62 + / - 0.11 for ouabain vs 0.45 + / - 0.09 for oxidized ouabain ( p & lt ; 0.05 ) , but the inotropic to toxic dose ratios were not different .
	manualset3
162045	2	411985	7	NULL	NULL	0	NULL	toxic dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of toxic to lethal doses was 0.62 + / - 0.11 for ouabain vs 0.45 + / - 0.09 for oxidized ouabain ( p & lt ; 0.05 ) , but the inotropic to toxic dose ratios were not different .
	manualset3
162046	3	411985	7	NULL	NULL	0	NULL	lethal doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of toxic to lethal doses was 0.62 + / - 0.11 for ouabain vs 0.45 + / - 0.09 for oxidized ouabain ( p & lt ; 0.05 ) , but the inotropic to toxic dose ratios were not different .
	manualset3
162047	4	411985	7	NULL	NULL	0	NULL	0.62 + / - 0.11	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of toxic to lethal doses was 0.62 + / - 0.11 for ouabain vs 0.45 + / - 0.09 for oxidized ouabain ( p & lt ; 0.05 ) , but the inotropic to toxic dose ratios were not different .
	manualset3
162048	5	411985	7	NULL	NULL	0	NULL	ouabain	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of toxic to lethal doses was 0.62 + / - 0.11 for ouabain vs 0.45 + / - 0.09 for oxidized ouabain ( p & lt ; 0.05 ) , but the inotropic to toxic dose ratios were not different .
	manualset3
162049	6	411985	7	NULL	NULL	0	NULL	0.45 + / - 0.09	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of toxic to lethal doses was 0.62 + / - 0.11 for ouabain vs 0.45 + / - 0.09 for oxidized ouabain ( p & lt ; 0.05 ) , but the inotropic to toxic dose ratios were not different .
	manualset3
162050	7	411985	7	NULL	NULL	0	NULL	oxidized ouabain	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of toxic to lethal doses was 0.62 + / - 0.11 for ouabain vs 0.45 + / - 0.09 for oxidized ouabain ( p & lt ; 0.05 ) , but the inotropic to toxic dose ratios were not different .
	manualset3
162051	8	411985	7	NULL	NULL	NULL	NULL	inotropic dose	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ratio of toxic to lethal doses was 0.62 + / - 0.11 for ouabain vs 0.45 + / - 0.09 for oxidized ouabain ( p & lt ; 0.05 ) , but the inotropic to toxic dose ratios were not different .
	manualset3
162052	9	411985	7	NULL	NULL	0	NULL	toxic dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of toxic to lethal doses was 0.62 + / - 0.11 for ouabain vs 0.45 + / - 0.09 for oxidized ouabain ( p & lt ; 0.05 ) , but the inotropic to toxic dose ratios were not different .
	manualset3
162053	10	411985	7	NULL	NULL	NULL	NULL	ratios	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ratio of toxic to lethal doses was 0.62 + / - 0.11 for ouabain vs 0.45 + / - 0.09 for oxidized ouabain ( p & lt ; 0.05 ) , but the inotropic to toxic dose ratios were not different .
	manualset3
162054	1	411986	7	NULL	NULL	0	NULL	ratios 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratios between the amplitudes of the second and first evoked potentials ( EPs or fEPSPs ) were taken as measures of the inhibitory capacity in the MI ipsilateral or contralateral to the nerve injury .
	manualset3
162055	2	411986	7	NULL	NULL	0	NULL	amplitudes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratios between the amplitudes of the second and first evoked potentials ( EPs or fEPSPs ) were taken as measures of the inhibitory capacity in the MI ipsilateral or contralateral to the nerve injury .
	manualset3
162056	3	411986	7	NULL	NULL	0	NULL	second evoked potential	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratios between the amplitudes of the second and first evoked potentials ( EPs or fEPSPs ) were taken as measures of the inhibitory capacity in the MI ipsilateral or contralateral to the nerve injury .
	manualset3
162057	4	411986	7	NULL	NULL	0	NULL	first evoked potentials	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratios between the amplitudes of the second and first evoked potentials ( EPs or fEPSPs ) were taken as measures of the inhibitory capacity in the MI ipsilateral or contralateral to the nerve injury .
	manualset3
162058	5	411986	7	NULL	NULL	0	NULL	EPs or fEPSPs	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratios between the amplitudes of the second and first evoked potentials ( EPs or fEPSPs ) were taken as measures of the inhibitory capacity in the MI ipsilateral or contralateral to the nerve injury .
	manualset3
162059	6	411986	7	NULL	NULL	0	NULL	measures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratios between the amplitudes of the second and first evoked potentials ( EPs or fEPSPs ) were taken as measures of the inhibitory capacity in the MI ipsilateral or contralateral to the nerve injury .
	manualset3
162060	7	411986	7	NULL	NULL	0	NULL	inhibitory capacity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratios between the amplitudes of the second and first evoked potentials ( EPs or fEPSPs ) were taken as measures of the inhibitory capacity in the MI ipsilateral or contralateral to the nerve injury .
	manualset3
162061	8	411986	7	NULL	NULL	0	NULL	MI ipsilateral	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratios between the amplitudes of the second and first evoked potentials ( EPs or fEPSPs ) were taken as measures of the inhibitory capacity in the MI ipsilateral or contralateral to the nerve injury .
	manualset3
162062	9	411986	7	NULL	NULL	0	NULL	MI contralateral 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratios between the amplitudes of the second and first evoked potentials ( EPs or fEPSPs ) were taken as measures of the inhibitory capacity in the MI ipsilateral or contralateral to the nerve injury .
	manualset3
162063	10	411986	7	NULL	NULL	0	NULL	nerve injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratios between the amplitudes of the second and first evoked potentials ( EPs or fEPSPs ) were taken as measures of the inhibitory capacity in the MI ipsilateral or contralateral to the nerve injury .
	manualset3
162064	1	411987	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The rats previously receiving morphine drank significantly less saccharin-water solution than did the rats receiving nicotine or saline injections .
	manualset3
162065	2	411987	7	NULL	NULL	0	NULL	morphine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The rats previously receiving morphine drank significantly less saccharin-water solution than did the rats receiving nicotine or saline injections .
	manualset3
162066	3	411987	7	NULL	NULL	0	NULL	saccharin-water solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The rats previously receiving morphine drank significantly less saccharin-water solution than did the rats receiving nicotine or saline injections .
	manualset3
162067	4	411987	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The rats previously receiving morphine drank significantly less saccharin-water solution than did the rats receiving nicotine or saline injections .
	manualset3
162068	5	411987	7	NULL	NULL	NULL	NULL	nicotine injections	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The rats previously receiving morphine drank significantly less saccharin-water solution than did the rats receiving nicotine or saline injections .
	manualset3
162069	6	411987	7	NULL	NULL	0	NULL	saline injections	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The rats previously receiving morphine drank significantly less saccharin-water solution than did the rats receiving nicotine or saline injections .
	manualset3
162070	1	411988	7	NULL	NULL	0	NULL	Abnormal Liver Function Investigations Evaluation ( ALFIE )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Abnormal Liver Function Investigations Evaluation ( ALFIE ) .
	manualset3
162071	1	411989	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The rats were sacrificed immediately after imaging , and the wet-to-dry ratio of the lung was measured .
	manualset3
162072	2	411989	7	NULL	NULL	0	NULL	imaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rats were sacrificed immediately after imaging , and the wet-to-dry ratio of the lung was measured .
	manualset3
162073	3	411989	7	NULL	NULL	0	NULL	wet-to-dry ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rats were sacrificed immediately after imaging , and the wet-to-dry ratio of the lung was measured .
	manualset3
162074	4	411989	7	NULL	NULL	0	NULL	 lung	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The rats were sacrificed immediately after imaging , and the wet-to-dry ratio of the lung was measured .
	manualset3
162075	1	411990	7	NULL	NULL	0	NULL	 reaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction between the Ni ( + ) cation and H ( 2 ) S is studied by considering both the doublet ground state and the lowest-lying quartet state .
	manualset3
162076	2	411990	7	NULL	NULL	0	NULL	Ni ( + ) cation	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction between the Ni ( + ) cation and H ( 2 ) S is studied by considering both the doublet ground state and the lowest-lying quartet state .
	manualset3
162077	3	411990	7	NULL	NULL	0	NULL	 H ( 2 ) S 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction between the Ni ( + ) cation and H ( 2 ) S is studied by considering both the doublet ground state and the lowest-lying quartet state .
	manualset3
162078	4	411990	7	NULL	NULL	NULL	NULL	 doublet ground state	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reaction between the Ni ( + ) cation and H ( 2 ) S is studied by considering both the doublet ground state and the lowest-lying quartet state .
	manualset3
162079	5	411990	7	NULL	NULL	NULL	NULL	lowest-lying quartet state	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reaction between the Ni ( + ) cation and H ( 2 ) S is studied by considering both the doublet ground state and the lowest-lying quartet state .
	manualset3
162080	1	411991	7	NULL	NULL	NULL	NULL	reaction mixture	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reaction mixture included purified spinach PSI reaction centers , sodium ascorbate and spinach plastocyanin .
	manualset3
162081	2	411991	7	NULL	NULL	NULL	NULL	purified spinach PSI reaction centers	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reaction mixture included purified spinach PSI reaction centers , sodium ascorbate and spinach plastocyanin .
	manualset3
162082	3	411991	7	NULL	NULL	0	NULL	sodium ascorbate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction mixture included purified spinach PSI reaction centers , sodium ascorbate and spinach plastocyanin .
	manualset3
162083	4	411991	7	NULL	NULL	0	NULL	spinach plastocyanin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction mixture included purified spinach PSI reaction centers , sodium ascorbate and spinach plastocyanin .
	manualset3
162084	1	411992	7	NULL	NULL	0	NULL	reaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction of anti-mony ( III ) chloride , 4 , 4 ' - bipyridine ( 4 , 4 ' - bipy ) and pyridine-2 , 6 - dicarboxylic acid ( pydcH ( 2 ) ) , in a 1 : 2 : 2 molar ratio in an aqueous solution , resulted in the formation of the title centrosymmetric disordered mixed-valence Sb ( III ) / Sb ( V ) compound , ( C ( 10 ) H ( 9 ) N ( 2 ) ) ( 2 ) ( Sb ( 2 ) ( C ( 7 ) H ( 3 ) NO ( 4 ) ) ( 2 ) ( OH ) ( 6 ) ) 8H ( 2 ) O or ( 4 , 4 ' - bipyH ) ( 2 ) ( Sb ( pydc ) ( OH ) ( 2 ) ( - OH ) ) ( 2 ) 8H ( 2 ) O. The seven donor atoms of the ( pydc ) ( 2 - ) groups and the hydroxido ligands form a distorted penta-gonal-bipyramidal arrangement around the Sb ( III ) / Sb ( V ) centers .
	manualset3
162085	2	411992	7	NULL	NULL	0	NULL	anti-mony ( III ) chloride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction of anti-mony ( III ) chloride , 4 , 4 ' - bipyridine ( 4 , 4 ' - bipy ) and pyridine-2 , 6 - dicarboxylic acid ( pydcH ( 2 ) ) , in a 1 : 2 : 2 molar ratio in an aqueous solution , resulted in the formation of the title centrosymmetric disordered mixed-valence Sb ( III ) / Sb ( V ) compound , ( C ( 10 ) H ( 9 ) N ( 2 ) ) ( 2 ) ( Sb ( 2 ) ( C ( 7 ) H ( 3 ) NO ( 4 ) ) ( 2 ) ( OH ) ( 6 ) ) 8H ( 2 ) O or ( 4 , 4 ' - bipyH ) ( 2 ) ( Sb ( pydc ) ( OH ) ( 2 ) ( - OH ) ) ( 2 ) 8H ( 2 ) O. The seven donor atoms of the ( pydc ) ( 2 - ) groups and the hydroxido ligands form a distorted penta-gonal-bipyramidal arrangement around the Sb ( III ) / Sb ( V ) centers .
	manualset3
162086	3	411992	7	NULL	NULL	0	NULL	 4 , 4 ' - bipyridine ( 4 , 4 ' - bipy ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction of anti-mony ( III ) chloride , 4 , 4 ' - bipyridine ( 4 , 4 ' - bipy ) and pyridine-2 , 6 - dicarboxylic acid ( pydcH ( 2 ) ) , in a 1 : 2 : 2 molar ratio in an aqueous solution , resulted in the formation of the title centrosymmetric disordered mixed-valence Sb ( III ) / Sb ( V ) compound , ( C ( 10 ) H ( 9 ) N ( 2 ) ) ( 2 ) ( Sb ( 2 ) ( C ( 7 ) H ( 3 ) NO ( 4 ) ) ( 2 ) ( OH ) ( 6 ) ) 8H ( 2 ) O or ( 4 , 4 ' - bipyH ) ( 2 ) ( Sb ( pydc ) ( OH ) ( 2 ) ( - OH ) ) ( 2 ) 8H ( 2 ) O. The seven donor atoms of the ( pydc ) ( 2 - ) groups and the hydroxido ligands form a distorted penta-gonal-bipyramidal arrangement around the Sb ( III ) / Sb ( V ) centers .
	manualset3
162087	4	411992	7	NULL	NULL	0	NULL	pyridine-2 , 6 - dicarboxylic acid ( pydcH ( 2 ) )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction of anti-mony ( III ) chloride , 4 , 4 ' - bipyridine ( 4 , 4 ' - bipy ) and pyridine-2 , 6 - dicarboxylic acid ( pydcH ( 2 ) ) , in a 1 : 2 : 2 molar ratio in an aqueous solution , resulted in the formation of the title centrosymmetric disordered mixed-valence Sb ( III ) / Sb ( V ) compound , ( C ( 10 ) H ( 9 ) N ( 2 ) ) ( 2 ) ( Sb ( 2 ) ( C ( 7 ) H ( 3 ) NO ( 4 ) ) ( 2 ) ( OH ) ( 6 ) ) 8H ( 2 ) O or ( 4 , 4 ' - bipyH ) ( 2 ) ( Sb ( pydc ) ( OH ) ( 2 ) ( - OH ) ) ( 2 ) 8H ( 2 ) O. The seven donor atoms of the ( pydc ) ( 2 - ) groups and the hydroxido ligands form a distorted penta-gonal-bipyramidal arrangement around the Sb ( III ) / Sb ( V ) centers .
	manualset3
162088	5	411992	7	NULL	NULL	0	NULL	1 : 2 : 2 molar ratio	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction of anti-mony ( III ) chloride , 4 , 4 ' - bipyridine ( 4 , 4 ' - bipy ) and pyridine-2 , 6 - dicarboxylic acid ( pydcH ( 2 ) ) , in a 1 : 2 : 2 molar ratio in an aqueous solution , resulted in the formation of the title centrosymmetric disordered mixed-valence Sb ( III ) / Sb ( V ) compound , ( C ( 10 ) H ( 9 ) N ( 2 ) ) ( 2 ) ( Sb ( 2 ) ( C ( 7 ) H ( 3 ) NO ( 4 ) ) ( 2 ) ( OH ) ( 6 ) ) 8H ( 2 ) O or ( 4 , 4 ' - bipyH ) ( 2 ) ( Sb ( pydc ) ( OH ) ( 2 ) ( - OH ) ) ( 2 ) 8H ( 2 ) O. The seven donor atoms of the ( pydc ) ( 2 - ) groups and the hydroxido ligands form a distorted penta-gonal-bipyramidal arrangement around the Sb ( III ) / Sb ( V ) centers .
	manualset3
162089	6	411992	7	NULL	NULL	0	NULL	aqueous solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction of anti-mony ( III ) chloride , 4 , 4 ' - bipyridine ( 4 , 4 ' - bipy ) and pyridine-2 , 6 - dicarboxylic acid ( pydcH ( 2 ) ) , in a 1 : 2 : 2 molar ratio in an aqueous solution , resulted in the formation of the title centrosymmetric disordered mixed-valence Sb ( III ) / Sb ( V ) compound , ( C ( 10 ) H ( 9 ) N ( 2 ) ) ( 2 ) ( Sb ( 2 ) ( C ( 7 ) H ( 3 ) NO ( 4 ) ) ( 2 ) ( OH ) ( 6 ) ) 8H ( 2 ) O or ( 4 , 4 ' - bipyH ) ( 2 ) ( Sb ( pydc ) ( OH ) ( 2 ) ( - OH ) ) ( 2 ) 8H ( 2 ) O. The seven donor atoms of the ( pydc ) ( 2 - ) groups and the hydroxido ligands form a distorted penta-gonal-bipyramidal arrangement around the Sb ( III ) / Sb ( V ) centers .
	manualset3
162090	7	411992	7	NULL	NULL	0	NULL	formation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction of anti-mony ( III ) chloride , 4 , 4 ' - bipyridine ( 4 , 4 ' - bipy ) and pyridine-2 , 6 - dicarboxylic acid ( pydcH ( 2 ) ) , in a 1 : 2 : 2 molar ratio in an aqueous solution , resulted in the formation of the title centrosymmetric disordered mixed-valence Sb ( III ) / Sb ( V ) compound , ( C ( 10 ) H ( 9 ) N ( 2 ) ) ( 2 ) ( Sb ( 2 ) ( C ( 7 ) H ( 3 ) NO ( 4 ) ) ( 2 ) ( OH ) ( 6 ) ) 8H ( 2 ) O or ( 4 , 4 ' - bipyH ) ( 2 ) ( Sb ( pydc ) ( OH ) ( 2 ) ( - OH ) ) ( 2 ) 8H ( 2 ) O. The seven donor atoms of the ( pydc ) ( 2 - ) groups and the hydroxido ligands form a distorted penta-gonal-bipyramidal arrangement around the Sb ( III ) / Sb ( V ) centers .
	manualset3
162092	9	411992	7	NULL	NULL	NULL	NULL	title centrosymmetric disordered mixed-valence Sb ( III ) / Sb ( V ) compound	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reaction of anti-mony ( III ) chloride , 4 , 4 ' - bipyridine ( 4 , 4 ' - bipy ) and pyridine-2 , 6 - dicarboxylic acid ( pydcH ( 2 ) ) , in a 1 : 2 : 2 molar ratio in an aqueous solution , resulted in the formation of the title centrosymmetric disordered mixed-valence Sb ( III ) / Sb ( V ) compound , ( C ( 10 ) H ( 9 ) N ( 2 ) ) ( 2 ) ( Sb ( 2 ) ( C ( 7 ) H ( 3 ) NO ( 4 ) ) ( 2 ) ( OH ) ( 6 ) ) 8H ( 2 ) O or ( 4 , 4 ' - bipyH ) ( 2 ) ( Sb ( pydc ) ( OH ) ( 2 ) ( - OH ) ) ( 2 ) 8H ( 2 ) O. The seven donor atoms of the ( pydc ) ( 2 - ) groups and the hydroxido ligands form a distorted penta-gonal-bipyramidal arrangement around the Sb ( III ) / Sb ( V ) centers .
	manualset3
162093	10	411992	7	NULL	NULL	NULL	NULL	( C ( 10 ) H ( 9 ) N ( 2 ) ) ( 2 ) ( Sb ( 2 ) ( C ( 7 ) H ( 3 ) NO ( 4 ) ) ( 2 ) ( OH ) ( 6 ) ) 8H ( 2 ) O 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reaction of anti-mony ( III ) chloride , 4 , 4 ' - bipyridine ( 4 , 4 ' - bipy ) and pyridine-2 , 6 - dicarboxylic acid ( pydcH ( 2 ) ) , in a 1 : 2 : 2 molar ratio in an aqueous solution , resulted in the formation of the title centrosymmetric disordered mixed-valence Sb ( III ) / Sb ( V ) compound , ( C ( 10 ) H ( 9 ) N ( 2 ) ) ( 2 ) ( Sb ( 2 ) ( C ( 7 ) H ( 3 ) NO ( 4 ) ) ( 2 ) ( OH ) ( 6 ) ) 8H ( 2 ) O or ( 4 , 4 ' - bipyH ) ( 2 ) ( Sb ( pydc ) ( OH ) ( 2 ) ( - OH ) ) ( 2 ) 8H ( 2 ) O. The seven donor atoms of the ( pydc ) ( 2 - ) groups and the hydroxido ligands form a distorted penta-gonal-bipyramidal arrangement around the Sb ( III ) / Sb ( V ) centers .
	manualset3
162094	11	411992	7	NULL	NULL	NULL	NULL	( 4 , 4 ' - bipyH ) ( 2 ) ( Sb ( pydc ) ( OH ) ( 2 ) ( - OH ) ) ( 2 ) 8H ( 2 ) O	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reaction of anti-mony ( III ) chloride , 4 , 4 ' - bipyridine ( 4 , 4 ' - bipy ) and pyridine-2 , 6 - dicarboxylic acid ( pydcH ( 2 ) ) , in a 1 : 2 : 2 molar ratio in an aqueous solution , resulted in the formation of the title centrosymmetric disordered mixed-valence Sb ( III ) / Sb ( V ) compound , ( C ( 10 ) H ( 9 ) N ( 2 ) ) ( 2 ) ( Sb ( 2 ) ( C ( 7 ) H ( 3 ) NO ( 4 ) ) ( 2 ) ( OH ) ( 6 ) ) 8H ( 2 ) O or ( 4 , 4 ' - bipyH ) ( 2 ) ( Sb ( pydc ) ( OH ) ( 2 ) ( - OH ) ) ( 2 ) 8H ( 2 ) O. The seven donor atoms of the ( pydc ) ( 2 - ) groups and the hydroxido ligands form a distorted penta-gonal-bipyramidal arrangement around the Sb ( III ) / Sb ( V ) centers .
	manualset3
162095	12	411992	7	NULL	NULL	0	NULL	seven donor atoms	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction of anti-mony ( III ) chloride , 4 , 4 ' - bipyridine ( 4 , 4 ' - bipy ) and pyridine-2 , 6 - dicarboxylic acid ( pydcH ( 2 ) ) , in a 1 : 2 : 2 molar ratio in an aqueous solution , resulted in the formation of the title centrosymmetric disordered mixed-valence Sb ( III ) / Sb ( V ) compound , ( C ( 10 ) H ( 9 ) N ( 2 ) ) ( 2 ) ( Sb ( 2 ) ( C ( 7 ) H ( 3 ) NO ( 4 ) ) ( 2 ) ( OH ) ( 6 ) ) 8H ( 2 ) O or ( 4 , 4 ' - bipyH ) ( 2 ) ( Sb ( pydc ) ( OH ) ( 2 ) ( - OH ) ) ( 2 ) 8H ( 2 ) O. The seven donor atoms of the ( pydc ) ( 2 - ) groups and the hydroxido ligands form a distorted penta-gonal-bipyramidal arrangement around the Sb ( III ) / Sb ( V ) centers .
	manualset3
162096	13	411992	7	NULL	NULL	0	NULL	( pydc ) ( 2 - ) groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction of anti-mony ( III ) chloride , 4 , 4 ' - bipyridine ( 4 , 4 ' - bipy ) and pyridine-2 , 6 - dicarboxylic acid ( pydcH ( 2 ) ) , in a 1 : 2 : 2 molar ratio in an aqueous solution , resulted in the formation of the title centrosymmetric disordered mixed-valence Sb ( III ) / Sb ( V ) compound , ( C ( 10 ) H ( 9 ) N ( 2 ) ) ( 2 ) ( Sb ( 2 ) ( C ( 7 ) H ( 3 ) NO ( 4 ) ) ( 2 ) ( OH ) ( 6 ) ) 8H ( 2 ) O or ( 4 , 4 ' - bipyH ) ( 2 ) ( Sb ( pydc ) ( OH ) ( 2 ) ( - OH ) ) ( 2 ) 8H ( 2 ) O. The seven donor atoms of the ( pydc ) ( 2 - ) groups and the hydroxido ligands form a distorted penta-gonal-bipyramidal arrangement around the Sb ( III ) / Sb ( V ) centers .
	manualset3
162097	14	411992	7	NULL	NULL	0	NULL	hydroxido ligands	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction of anti-mony ( III ) chloride , 4 , 4 ' - bipyridine ( 4 , 4 ' - bipy ) and pyridine-2 , 6 - dicarboxylic acid ( pydcH ( 2 ) ) , in a 1 : 2 : 2 molar ratio in an aqueous solution , resulted in the formation of the title centrosymmetric disordered mixed-valence Sb ( III ) / Sb ( V ) compound , ( C ( 10 ) H ( 9 ) N ( 2 ) ) ( 2 ) ( Sb ( 2 ) ( C ( 7 ) H ( 3 ) NO ( 4 ) ) ( 2 ) ( OH ) ( 6 ) ) 8H ( 2 ) O or ( 4 , 4 ' - bipyH ) ( 2 ) ( Sb ( pydc ) ( OH ) ( 2 ) ( - OH ) ) ( 2 ) 8H ( 2 ) O. The seven donor atoms of the ( pydc ) ( 2 - ) groups and the hydroxido ligands form a distorted penta-gonal-bipyramidal arrangement around the Sb ( III ) / Sb ( V ) centers .
	manualset3
162098	15	411992	7	NULL	NULL	0	NULL	distorted penta-gonal-bipyramidal arrangement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction of anti-mony ( III ) chloride , 4 , 4 ' - bipyridine ( 4 , 4 ' - bipy ) and pyridine-2 , 6 - dicarboxylic acid ( pydcH ( 2 ) ) , in a 1 : 2 : 2 molar ratio in an aqueous solution , resulted in the formation of the title centrosymmetric disordered mixed-valence Sb ( III ) / Sb ( V ) compound , ( C ( 10 ) H ( 9 ) N ( 2 ) ) ( 2 ) ( Sb ( 2 ) ( C ( 7 ) H ( 3 ) NO ( 4 ) ) ( 2 ) ( OH ) ( 6 ) ) 8H ( 2 ) O or ( 4 , 4 ' - bipyH ) ( 2 ) ( Sb ( pydc ) ( OH ) ( 2 ) ( - OH ) ) ( 2 ) 8H ( 2 ) O. The seven donor atoms of the ( pydc ) ( 2 - ) groups and the hydroxido ligands form a distorted penta-gonal-bipyramidal arrangement around the Sb ( III ) / Sb ( V ) centers .
	manualset3
162099	16	411992	7	NULL	NULL	0	NULL	Sb ( III ) / Sb ( V ) centers 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction of anti-mony ( III ) chloride , 4 , 4 ' - bipyridine ( 4 , 4 ' - bipy ) and pyridine-2 , 6 - dicarboxylic acid ( pydcH ( 2 ) ) , in a 1 : 2 : 2 molar ratio in an aqueous solution , resulted in the formation of the title centrosymmetric disordered mixed-valence Sb ( III ) / Sb ( V ) compound , ( C ( 10 ) H ( 9 ) N ( 2 ) ) ( 2 ) ( Sb ( 2 ) ( C ( 7 ) H ( 3 ) NO ( 4 ) ) ( 2 ) ( OH ) ( 6 ) ) 8H ( 2 ) O or ( 4 , 4 ' - bipyH ) ( 2 ) ( Sb ( pydc ) ( OH ) ( 2 ) ( - OH ) ) ( 2 ) 8H ( 2 ) O. The seven donor atoms of the ( pydc ) ( 2 - ) groups and the hydroxido ligands form a distorted penta-gonal-bipyramidal arrangement around the Sb ( III ) / Sb ( V ) centers .
	manualset3
162100	1	411993	7	NULL	NULL	0	NULL	 reaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction provided bis triazolyl substituted quinolines when performed in water in the presence of Et ( 3 ) N. A number of the compounds synthesized showed promising anti-proliferative properties when tested in vitro especially against breast cancer cells .
	manualset3
162101	2	411993	7	NULL	NULL	0	NULL	bis triazolyl substituted quinolines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction provided bis triazolyl substituted quinolines when performed in water in the presence of Et ( 3 ) N. A number of the compounds synthesized showed promising anti-proliferative properties when tested in vitro especially against breast cancer cells .
	manualset3
162102	3	411993	7	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction provided bis triazolyl substituted quinolines when performed in water in the presence of Et ( 3 ) N. A number of the compounds synthesized showed promising anti-proliferative properties when tested in vitro especially against breast cancer cells .
	manualset3
162103	4	411993	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction provided bis triazolyl substituted quinolines when performed in water in the presence of Et ( 3 ) N. A number of the compounds synthesized showed promising anti-proliferative properties when tested in vitro especially against breast cancer cells .
	manualset3
162104	5	411993	7	NULL	NULL	0	NULL	Et ( 3 ) N	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction provided bis triazolyl substituted quinolines when performed in water in the presence of Et ( 3 ) N. A number of the compounds synthesized showed promising anti-proliferative properties when tested in vitro especially against breast cancer cells .
	manualset3
162105	6	411993	7	NULL	NULL	0	NULL	compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction provided bis triazolyl substituted quinolines when performed in water in the presence of Et ( 3 ) N. A number of the compounds synthesized showed promising anti-proliferative properties when tested in vitro especially against breast cancer cells .
	manualset3
162106	7	411993	7	NULL	NULL	0	NULL	anti-proliferative properties	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction provided bis triazolyl substituted quinolines when performed in water in the presence of Et ( 3 ) N. A number of the compounds synthesized showed promising anti-proliferative properties when tested in vitro especially against breast cancer cells .
	manualset3
162107	8	411993	7	NULL	NULL	0	NULL	 breast cancer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction provided bis triazolyl substituted quinolines when performed in water in the presence of Et ( 3 ) N. A number of the compounds synthesized showed promising anti-proliferative properties when tested in vitro especially against breast cancer cells .
	manualset3
162108	1	411994	7	NULL	NULL	0	NULL	reactivation phenomenon	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The reactivation phenomenon is hardly observed when incubating HSL with compound 9368 .
	manualset3
162109	2	411994	7	NULL	NULL	0	NULL	HSL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The reactivation phenomenon is hardly observed when incubating HSL with compound 9368 .
	manualset3
162110	3	411994	7	NULL	NULL	0	NULL	compound 9368	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reactivation phenomenon is hardly observed when incubating HSL with compound 9368 .
	manualset3
162111	1	411995	7	NULL	NULL	0	NULL	reactivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The reactivity of JC1 was sharply reduced by anti-L3T4 ( CD4 ) or by anti-I-Ab monoclonal antibody .
	manualset3
162112	2	411995	7	NULL	NULL	0	NULL	JC1	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reactivity of JC1 was sharply reduced by anti-L3T4 ( CD4 ) or by anti-I-Ab monoclonal antibody .
	manualset3
162113	3	411995	7	NULL	NULL	0	NULL	anti-L3T4 ( CD4 ) antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The reactivity of JC1 was sharply reduced by anti-L3T4 ( CD4 ) or by anti-I-Ab monoclonal antibody .
	manualset3
162114	4	411995	7	NULL	NULL	0	NULL	anti-I-Ab monoclonal antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The reactivity of JC1 was sharply reduced by anti-L3T4 ( CD4 ) or by anti-I-Ab monoclonal antibody .
	manualset3
162115	1	411996	7	NULL	NULL	0	NULL	reactor 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The reactor exhibited a selectivity for CO2 versus N2 of 1400 : 1 and CO2 versus O2 is 866 : 1 .
	manualset3
162116	2	411996	7	NULL	NULL	0	NULL	 selectivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The reactor exhibited a selectivity for CO2 versus N2 of 1400 : 1 and CO2 versus O2 is 866 : 1 .
	manualset3
162117	3	411996	7	NULL	NULL	0	NULL	CO2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reactor exhibited a selectivity for CO2 versus N2 of 1400 : 1 and CO2 versus O2 is 866 : 1 .
	manualset3
162118	4	411996	7	NULL	NULL	0	NULL	N2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reactor exhibited a selectivity for CO2 versus N2 of 1400 : 1 and CO2 versus O2 is 866 : 1 .
	manualset3
162119	5	411996	7	NULL	NULL	0	NULL	1400 : 1	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The reactor exhibited a selectivity for CO2 versus N2 of 1400 : 1 and CO2 versus O2 is 866 : 1 .
	manualset3
162120	6	411996	7	NULL	NULL	0	NULL	CO2 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reactor exhibited a selectivity for CO2 versus N2 of 1400 : 1 and CO2 versus O2 is 866 : 1 .
	manualset3
162121	7	411996	7	NULL	NULL	0	NULL	O2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reactor exhibited a selectivity for CO2 versus N2 of 1400 : 1 and CO2 versus O2 is 866 : 1 .
	manualset3
162122	8	411996	7	NULL	NULL	0	NULL	866 : 1	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The reactor exhibited a selectivity for CO2 versus N2 of 1400 : 1 and CO2 versus O2 is 866 : 1 .
	manualset3
162123	1	411997	7	NULL	NULL	0	NULL	Abnormal adaptations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Abnormal adaptations to stress and impaired cardiovascular function in mice lacking corticotropin-releasing hormone receptor-2 .
	manualset3
162125	3	411997	7	NULL	NULL	0	NULL	impaired cardiovascular function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Abnormal adaptations to stress and impaired cardiovascular function in mice lacking corticotropin-releasing hormone receptor-2 .
	manualset3
162126	4	411997	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Abnormal adaptations to stress and impaired cardiovascular function in mice lacking corticotropin-releasing hormone receptor-2 .
	manualset3
162127	5	411997	7	NULL	NULL	0	NULL	corticotropin-releasing hormone receptor-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Abnormal adaptations to stress and impaired cardiovascular function in mice lacking corticotropin-releasing hormone receptor-2 .
	manualset3
162902	2	411997	7	NULL	NULL	0	NULL	stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Abnormal adaptations to stress and impaired cardiovascular function in mice lacking corticotropin-releasing hormone receptor-2 .
	manualset3
162128	1	411998	7	NULL	NULL	0	NULL	reactor 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The reactor was operated for 160 days at different chemical oxygen demand ( COD ) / sulfate ratios , hydraulic retention times ( HRT ) , pH , and metal concentrations to study the robustness of the process .
	manualset3
162129	2	411998	7	NULL	NULL	0	NULL	160 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The reactor was operated for 160 days at different chemical oxygen demand ( COD ) / sulfate ratios , hydraulic retention times ( HRT ) , pH , and metal concentrations to study the robustness of the process .
	manualset3
162130	3	411998	7	NULL	NULL	0	NULL	chemical oxygen demand ( COD ) / sulfate ratios	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The reactor was operated for 160 days at different chemical oxygen demand ( COD ) / sulfate ratios , hydraulic retention times ( HRT ) , pH , and metal concentrations to study the robustness of the process .
	manualset3
162131	4	411998	7	NULL	NULL	0	NULL	hydraulic retention times ( HRT )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The reactor was operated for 160 days at different chemical oxygen demand ( COD ) / sulfate ratios , hydraulic retention times ( HRT ) , pH , and metal concentrations to study the robustness of the process .
	manualset3
162132	5	411998	7	NULL	NULL	0	NULL	pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The reactor was operated for 160 days at different chemical oxygen demand ( COD ) / sulfate ratios , hydraulic retention times ( HRT ) , pH , and metal concentrations to study the robustness of the process .
	manualset3
162133	6	411998	7	NULL	NULL	0	NULL	metal concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The reactor was operated for 160 days at different chemical oxygen demand ( COD ) / sulfate ratios , hydraulic retention times ( HRT ) , pH , and metal concentrations to study the robustness of the process .
	manualset3
162134	7	411998	7	NULL	NULL	0	NULL	process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The reactor was operated for 160 days at different chemical oxygen demand ( COD ) / sulfate ratios , hydraulic retention times ( HRT ) , pH , and metal concentrations to study the robustness of the process .
	manualset3
162135	1	411999	7	NULL	NULL	0	NULL	real-time reflectance changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The real-time reflectance changes induced by discrete variations in glucose concentration has been revealed and analyzed .
	manualset3
162136	2	411999	7	NULL	NULL	0	NULL	discrete variations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The real-time reflectance changes induced by discrete variations in glucose concentration has been revealed and analyzed .
	manualset3
162137	3	411999	7	NULL	NULL	0	NULL	 glucose concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The real-time reflectance changes induced by discrete variations in glucose concentration has been revealed and analyzed .
	manualset3
162138	1	412000	7	NULL	NULL	NULL	NULL	real benefits 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The real benefits of extracorporeal membrane oxygenation are not defined yet .
	manualset3
162139	2	412000	7	NULL	NULL	NULL	NULL	extracorporeal membrane oxygenation 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The real benefits of extracorporeal membrane oxygenation are not defined yet .
	manualset3
162141	1	412001	7	NULL	NULL	NULL	NULL	 challenge	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The real challenge in healthcare marketing today is managing markets , focusing on selected groups of customers rather than on the organization or its services .
	manualset3
162142	2	412001	7	NULL	NULL	0	NULL	healthcare marketing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The real challenge in healthcare marketing today is managing markets , focusing on selected groups of customers rather than on the organization or its services .
	manualset3
162143	3	412001	7	NULL	NULL	NULL	NULL	today	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The real challenge in healthcare marketing today is managing markets , focusing on selected groups of customers rather than on the organization or its services .
	manualset3
162144	4	412001	7	NULL	NULL	0	NULL	markets	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The real challenge in healthcare marketing today is managing markets , focusing on selected groups of customers rather than on the organization or its services .
	manualset3
162145	5	412001	7	NULL	NULL	0	NULL	groups of customers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The real challenge in healthcare marketing today is managing markets , focusing on selected groups of customers rather than on the organization or its services .
	manualset3
162146	6	412001	7	NULL	NULL	0	NULL	organization	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The real challenge in healthcare marketing today is managing markets , focusing on selected groups of customers rather than on the organization or its services .
	manualset3
162147	7	412001	7	NULL	NULL	0	NULL	services	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The real challenge in healthcare marketing today is managing markets , focusing on selected groups of customers rather than on the organization or its services .
	manualset3
162148	1	412002	7	NULL	NULL	0	NULL	reality	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The reality of enforced treatment and the very real influence treaters have on the lives of their patients supports a particular and salient transferential experience of the therapist as an authority figure who is generally also seen as harsh and arbitrary .
	manualset3
162149	2	412002	7	NULL	NULL	0	NULL	enforced treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The reality of enforced treatment and the very real influence treaters have on the lives of their patients supports a particular and salient transferential experience of the therapist as an authority figure who is generally also seen as harsh and arbitrary .
	manualset3
162150	3	412002	7	NULL	NULL	0	NULL	treaters	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The reality of enforced treatment and the very real influence treaters have on the lives of their patients supports a particular and salient transferential experience of the therapist as an authority figure who is generally also seen as harsh and arbitrary .
	manualset3
162152	5	412002	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The reality of enforced treatment and the very real influence treaters have on the lives of their patients supports a particular and salient transferential experience of the therapist as an authority figure who is generally also seen as harsh and arbitrary .
	manualset3
162153	6	412002	7	NULL	NULL	NULL	NULL	transferential experience	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reality of enforced treatment and the very real influence treaters have on the lives of their patients supports a particular and salient transferential experience of the therapist as an authority figure who is generally also seen as harsh and arbitrary .
	manualset3
162154	7	412002	7	NULL	NULL	0	NULL	 therapist	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The reality of enforced treatment and the very real influence treaters have on the lives of their patients supports a particular and salient transferential experience of the therapist as an authority figure who is generally also seen as harsh and arbitrary .
	manualset3
162155	8	412002	7	NULL	NULL	0	NULL	authority figure	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The reality of enforced treatment and the very real influence treaters have on the lives of their patients supports a particular and salient transferential experience of the therapist as an authority figure who is generally also seen as harsh and arbitrary .
	manualset3
162903	9	412002	7	NULL	NULL	0	NULL	influence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The reality of enforced treatment and the very real influence treaters have on the lives of their patients supports a particular and salient transferential experience of the therapist as an authority figure who is generally also seen as harsh and arbitrary .
	manualset3
162904	4	412002	7	NULL	NULL	0	NULL	lives 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The reality of enforced treatment and the very real influence treaters have on the lives of their patients supports a particular and salient transferential experience of the therapist as an authority figure who is generally also seen as harsh and arbitrary .
	manualset3
162156	1	412003	7	NULL	NULL	NULL	NULL	 rearrangement 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The rearrangement results in fusion of the RUNX1 ( also known as AML1 ) and CBFA2T1 ( also known as ETO ) genes , generating a 5 ` RUNX1/3 ` CBFA2T1 transcriptionally active fusion gene on derivative chromosome 8 , but some cases with ins ( 21 ; 8 ) and ins ( 8 ; 21 ) have been observed .
	manualset3
162157	2	412003	7	NULL	NULL	0	NULL	fusion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The rearrangement results in fusion of the RUNX1 ( also known as AML1 ) and CBFA2T1 ( also known as ETO ) genes , generating a 5 ` RUNX1/3 ` CBFA2T1 transcriptionally active fusion gene on derivative chromosome 8 , but some cases with ins ( 21 ; 8 ) and ins ( 8 ; 21 ) have been observed .
	manualset3
162158	3	412003	7	NULL	NULL	0	NULL	RUNX1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The rearrangement results in fusion of the RUNX1 ( also known as AML1 ) and CBFA2T1 ( also known as ETO ) genes , generating a 5 ` RUNX1/3 ` CBFA2T1 transcriptionally active fusion gene on derivative chromosome 8 , but some cases with ins ( 21 ; 8 ) and ins ( 8 ; 21 ) have been observed .
	manualset3
162159	4	412003	7	NULL	NULL	0	NULL	AML1 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The rearrangement results in fusion of the RUNX1 ( also known as AML1 ) and CBFA2T1 ( also known as ETO ) genes , generating a 5 ` RUNX1/3 ` CBFA2T1 transcriptionally active fusion gene on derivative chromosome 8 , but some cases with ins ( 21 ; 8 ) and ins ( 8 ; 21 ) have been observed .
	manualset3
162160	5	412003	7	NULL	NULL	0	NULL	CBFA2T1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The rearrangement results in fusion of the RUNX1 ( also known as AML1 ) and CBFA2T1 ( also known as ETO ) genes , generating a 5 ` RUNX1/3 ` CBFA2T1 transcriptionally active fusion gene on derivative chromosome 8 , but some cases with ins ( 21 ; 8 ) and ins ( 8 ; 21 ) have been observed .
	manualset3
162161	6	412003	7	NULL	NULL	0	NULL	ETO	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The rearrangement results in fusion of the RUNX1 ( also known as AML1 ) and CBFA2T1 ( also known as ETO ) genes , generating a 5 ` RUNX1/3 ` CBFA2T1 transcriptionally active fusion gene on derivative chromosome 8 , but some cases with ins ( 21 ; 8 ) and ins ( 8 ; 21 ) have been observed .
	manualset3
162162	7	412003	7	NULL	NULL	0	NULL	5 ` RUNX1/3 ` CBFA2T1 transcriptionally active fusion gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The rearrangement results in fusion of the RUNX1 ( also known as AML1 ) and CBFA2T1 ( also known as ETO ) genes , generating a 5 ` RUNX1/3 ` CBFA2T1 transcriptionally active fusion gene on derivative chromosome 8 , but some cases with ins ( 21 ; 8 ) and ins ( 8 ; 21 ) have been observed .
	manualset3
162163	8	412003	7	NULL	NULL	0	NULL	chromosome 8	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The rearrangement results in fusion of the RUNX1 ( also known as AML1 ) and CBFA2T1 ( also known as ETO ) genes , generating a 5 ` RUNX1/3 ` CBFA2T1 transcriptionally active fusion gene on derivative chromosome 8 , but some cases with ins ( 21 ; 8 ) and ins ( 8 ; 21 ) have been observed .
	manualset3
162164	9	412003	7	NULL	NULL	NULL	NULL	cases	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The rearrangement results in fusion of the RUNX1 ( also known as AML1 ) and CBFA2T1 ( also known as ETO ) genes , generating a 5 ` RUNX1/3 ` CBFA2T1 transcriptionally active fusion gene on derivative chromosome 8 , but some cases with ins ( 21 ; 8 ) and ins ( 8 ; 21 ) have been observed .
	manualset3
162165	10	412003	7	NULL	NULL	0	NULL	 ins ( 21 ; 8 )	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The rearrangement results in fusion of the RUNX1 ( also known as AML1 ) and CBFA2T1 ( also known as ETO ) genes , generating a 5 ` RUNX1/3 ` CBFA2T1 transcriptionally active fusion gene on derivative chromosome 8 , but some cases with ins ( 21 ; 8 ) and ins ( 8 ; 21 ) have been observed .
	manualset3
162166	11	412003	7	NULL	NULL	0	NULL	 ins ( 8 ; 21 )	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The rearrangement results in fusion of the RUNX1 ( also known as AML1 ) and CBFA2T1 ( also known as ETO ) genes , generating a 5 ` RUNX1/3 ` CBFA2T1 transcriptionally active fusion gene on derivative chromosome 8 , but some cases with ins ( 21 ; 8 ) and ins ( 8 ; 21 ) have been observed .
	manualset3
162167	1	412004	7	NULL	NULL	0	NULL	reason 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The reason for the relatively long delay in LDV infection of anterior horn neurons is not known .
	manualset3
162168	2	412004	7	NULL	NULL	0	NULL	 long delay	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The reason for the relatively long delay in LDV infection of anterior horn neurons is not known .
	manualset3
162169	3	412004	7	NULL	NULL	0	NULL	LDV infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The reason for the relatively long delay in LDV infection of anterior horn neurons is not known .
	manualset3
162170	4	412004	7	NULL	NULL	0	NULL	anterior horn neurons	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The reason for the relatively long delay in LDV infection of anterior horn neurons is not known .
	manualset3
162171	1	412005	7	NULL	NULL	0	NULL	reason	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The reason for these disparities between numbers infected and numbers affected by illness is unknown , but presumably reflects host factor ( s ) .
	manualset3
162172	2	412005	7	NULL	NULL	NULL	NULL	numbers infected	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reason for these disparities between numbers infected and numbers affected by illness is unknown , but presumably reflects host factor ( s ) .
	manualset3
162173	3	412005	7	NULL	NULL	NULL	NULL	numbers affected	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reason for these disparities between numbers infected and numbers affected by illness is unknown , but presumably reflects host factor ( s ) .
	manualset3
162174	4	412005	7	NULL	NULL	0	NULL	 illness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The reason for these disparities between numbers infected and numbers affected by illness is unknown , but presumably reflects host factor ( s ) .
	manualset3
162175	5	412005	7	NULL	NULL	0	NULL	host factor ( s )	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The reason for these disparities between numbers infected and numbers affected by illness is unknown , but presumably reflects host factor ( s ) .
	manualset3
162176	1	412006	7	NULL	NULL	0	NULL	definition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent definition of minimally conscious state ( MCS ) , and possibly research advances ( e.g. , functional neuroimaging ) , may have lead to uncertainty regarding potential residual perception and may have influenced opinions of healthcare professionals .
	manualset3
162177	2	412006	7	NULL	NULL	0	NULL	minimally conscious state ( MCS )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent definition of minimally conscious state ( MCS ) , and possibly research advances ( e.g. , functional neuroimaging ) , may have lead to uncertainty regarding potential residual perception and may have influenced opinions of healthcare professionals .
	manualset3
162178	4	412006	7	NULL	NULL	NULL	NULL	functional neuroimaging	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The recent definition of minimally conscious state ( MCS ) , and possibly research advances ( e.g. , functional neuroimaging ) , may have lead to uncertainty regarding potential residual perception and may have influenced opinions of healthcare professionals .
	manualset3
162179	5	412006	7	NULL	NULL	NULL	NULL	potential residual perception	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The recent definition of minimally conscious state ( MCS ) , and possibly research advances ( e.g. , functional neuroimaging ) , may have lead to uncertainty regarding potential residual perception and may have influenced opinions of healthcare professionals .
	manualset3
162180	3	412006	7	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent definition of minimally conscious state ( MCS ) , and possibly research advances ( e.g. , functional neuroimaging ) , may have lead to uncertainty regarding potential residual perception and may have influenced opinions of healthcare professionals .
	manualset3
162181	6	412006	7	NULL	NULL	NULL	NULL	opinions	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The recent definition of minimally conscious state ( MCS ) , and possibly research advances ( e.g. , functional neuroimaging ) , may have lead to uncertainty regarding potential residual perception and may have influenced opinions of healthcare professionals .
	manualset3
162182	7	412006	7	NULL	NULL	0	NULL	healthcare professionals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent definition of minimally conscious state ( MCS ) , and possibly research advances ( e.g. , functional neuroimaging ) , may have lead to uncertainty regarding potential residual perception and may have influenced opinions of healthcare professionals .
	manualset3
162183	1	412007	7	NULL	NULL	0	NULL	developments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent developments of films that are ovenable in traditional as well as microwave ovens are critical to the further advancement of convenience meat items .
	manualset3
162184	2	412007	7	NULL	NULL	0	NULL	films	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent developments of films that are ovenable in traditional as well as microwave ovens are critical to the further advancement of convenience meat items .
	manualset3
162186	4	412007	7	NULL	NULL	0	NULL	microwave ovens	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent developments of films that are ovenable in traditional as well as microwave ovens are critical to the further advancement of convenience meat items .
	manualset3
162187	5	412007	7	NULL	NULL	0	NULL	advancement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent developments of films that are ovenable in traditional as well as microwave ovens are critical to the further advancement of convenience meat items .
	manualset3
162188	6	412007	7	NULL	NULL	0	NULL	convenience 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent developments of films that are ovenable in traditional as well as microwave ovens are critical to the further advancement of convenience meat items .
	manualset3
162189	7	412007	7	NULL	NULL	0	NULL	meat items	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent developments of films that are ovenable in traditional as well as microwave ovens are critical to the further advancement of convenience meat items .
	manualset3
162190	1	412008	7	NULL	NULL	0	NULL	discovery	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent discovery of an association between body composition , energy intake and the fat mass and obesity-associated ( FTO ) gene represents a promising new therapeutic target in obesity prevention .
	manualset3
162192	2	412008	7	NULL	NULL	0	NULL	association	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent discovery of an association between body composition , energy intake and the fat mass and obesity-associated ( FTO ) gene represents a promising new therapeutic target in obesity prevention .
	manualset3
162193	3	412008	7	NULL	NULL	NULL	NULL	body composition	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The recent discovery of an association between body composition , energy intake and the fat mass and obesity-associated ( FTO ) gene represents a promising new therapeutic target in obesity prevention .
	manualset3
162194	4	412008	7	NULL	NULL	0	NULL	energy intake	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent discovery of an association between body composition , energy intake and the fat mass and obesity-associated ( FTO ) gene represents a promising new therapeutic target in obesity prevention .
	manualset3
162195	5	412008	7	NULL	NULL	0	NULL	fat mass and obesity-associated ( FTO ) gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent discovery of an association between body composition , energy intake and the fat mass and obesity-associated ( FTO ) gene represents a promising new therapeutic target in obesity prevention .
	manualset3
162196	6	412008	7	NULL	NULL	0	NULL	new therapeutic target	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent discovery of an association between body composition , energy intake and the fat mass and obesity-associated ( FTO ) gene represents a promising new therapeutic target in obesity prevention .
	manualset3
162197	7	412008	7	NULL	NULL	0	NULL	obesity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent discovery of an association between body composition , energy intake and the fat mass and obesity-associated ( FTO ) gene represents a promising new therapeutic target in obesity prevention .
	manualset3
162198	8	412008	7	NULL	NULL	0	NULL	prevention	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent discovery of an association between body composition , energy intake and the fat mass and obesity-associated ( FTO ) gene represents a promising new therapeutic target in obesity prevention .
	manualset3
162199	1	412009	7	NULL	NULL	0	NULL	past	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent past has witnessed remarkable progress in finding genes for dystonia .
	manualset3
162200	2	412009	7	NULL	NULL	0	NULL	 progress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent past has witnessed remarkable progress in finding genes for dystonia .
	manualset3
162201	3	412009	7	NULL	NULL	0	NULL	genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent past has witnessed remarkable progress in finding genes for dystonia .
	manualset3
162202	4	412009	7	NULL	NULL	0	NULL	dystonia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent past has witnessed remarkable progress in finding genes for dystonia .
	manualset3
162203	1	412010	7	NULL	NULL	0	NULL	process analytical technology ( PAT ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent process analytical technology ( PAT ) initiative has put an increased focus on online sensors to generate process-relevant information in real time .
	manualset3
162204	2	412010	7	NULL	NULL	0	NULL	focus	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent process analytical technology ( PAT ) initiative has put an increased focus on online sensors to generate process-relevant information in real time .
	manualset3
162205	3	412010	7	NULL	NULL	0	NULL	online sensors	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent process analytical technology ( PAT ) initiative has put an increased focus on online sensors to generate process-relevant information in real time .
	manualset3
162206	4	412010	7	NULL	NULL	0	NULL	process-relevant information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent process analytical technology ( PAT ) initiative has put an increased focus on online sensors to generate process-relevant information in real time .
	manualset3
162207	5	412010	7	NULL	NULL	0	NULL	real time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent process analytical technology ( PAT ) initiative has put an increased focus on online sensors to generate process-relevant information in real time .
	manualset3
162208	1	412011	7	NULL	NULL	0	NULL	Abnormal immune responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Abnormal immune responses observed in microgravity may pose serious consequences , especially for the recent directions of NASA for long-term space missions to Moon , Mars and deep Space exploration .
	manualset3
162209	2	412011	7	NULL	NULL	0	NULL	microgravity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Abnormal immune responses observed in microgravity may pose serious consequences , especially for the recent directions of NASA for long-term space missions to Moon , Mars and deep Space exploration .
	manualset3
162210	3	412011	7	NULL	NULL	0	NULL	serious consequences	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Abnormal immune responses observed in microgravity may pose serious consequences , especially for the recent directions of NASA for long-term space missions to Moon , Mars and deep Space exploration .
	manualset3
162211	4	412011	7	NULL	NULL	0	NULL	directions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Abnormal immune responses observed in microgravity may pose serious consequences , especially for the recent directions of NASA for long-term space missions to Moon , Mars and deep Space exploration .
	manualset3
162212	5	412011	7	NULL	NULL	0	NULL	NASA	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Abnormal immune responses observed in microgravity may pose serious consequences , especially for the recent directions of NASA for long-term space missions to Moon , Mars and deep Space exploration .
	manualset3
162213	6	412011	7	NULL	NULL	0	NULL	long-term space missions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Abnormal immune responses observed in microgravity may pose serious consequences , especially for the recent directions of NASA for long-term space missions to Moon , Mars and deep Space exploration .
	manualset3
162214	7	412011	7	NULL	NULL	0	NULL	Moon	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Abnormal immune responses observed in microgravity may pose serious consequences , especially for the recent directions of NASA for long-term space missions to Moon , Mars and deep Space exploration .
	manualset3
162215	8	412011	7	NULL	NULL	0	NULL	Mars	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Abnormal immune responses observed in microgravity may pose serious consequences , especially for the recent directions of NASA for long-term space missions to Moon , Mars and deep Space exploration .
	manualset3
162216	9	412011	7	NULL	NULL	0	NULL	deep Space exploration	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Abnormal immune responses observed in microgravity may pose serious consequences , especially for the recent directions of NASA for long-term space missions to Moon , Mars and deep Space exploration .
	manualset3
162217	1	412012	7	NULL	NULL	0	NULL	publication 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent publication of the X-ray crystal structure for the enzymatic target of these compounds should facilitate the development of other new agents with enhanced activity that could improve both the diagnosis and treatment of neurological disorders .
	manualset3
162218	2	412012	7	NULL	NULL	0	NULL	 X-ray crystal structure	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent publication of the X-ray crystal structure for the enzymatic target of these compounds should facilitate the development of other new agents with enhanced activity that could improve both the diagnosis and treatment of neurological disorders .
	manualset3
162219	3	412012	7	NULL	NULL	0	NULL	enzymatic target	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent publication of the X-ray crystal structure for the enzymatic target of these compounds should facilitate the development of other new agents with enhanced activity that could improve both the diagnosis and treatment of neurological disorders .
	manualset3
162220	4	412012	7	NULL	NULL	0	NULL	compounds	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent publication of the X-ray crystal structure for the enzymatic target of these compounds should facilitate the development of other new agents with enhanced activity that could improve both the diagnosis and treatment of neurological disorders .
	manualset3
162221	5	412012	7	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent publication of the X-ray crystal structure for the enzymatic target of these compounds should facilitate the development of other new agents with enhanced activity that could improve both the diagnosis and treatment of neurological disorders .
	manualset3
162222	6	412012	7	NULL	NULL	NULL	NULL	new agents	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The recent publication of the X-ray crystal structure for the enzymatic target of these compounds should facilitate the development of other new agents with enhanced activity that could improve both the diagnosis and treatment of neurological disorders .
	manualset3
162223	7	412012	7	NULL	NULL	0	NULL	enhanced activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent publication of the X-ray crystal structure for the enzymatic target of these compounds should facilitate the development of other new agents with enhanced activity that could improve both the diagnosis and treatment of neurological disorders .
	manualset3
162224	8	412012	7	NULL	NULL	0	NULL	 diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent publication of the X-ray crystal structure for the enzymatic target of these compounds should facilitate the development of other new agents with enhanced activity that could improve both the diagnosis and treatment of neurological disorders .
	manualset3
162225	9	412012	7	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent publication of the X-ray crystal structure for the enzymatic target of these compounds should facilitate the development of other new agents with enhanced activity that could improve both the diagnosis and treatment of neurological disorders .
	manualset3
162226	10	412012	7	NULL	NULL	0	NULL	neurological disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent publication of the X-ray crystal structure for the enzymatic target of these compounds should facilitate the development of other new agents with enhanced activity that could improve both the diagnosis and treatment of neurological disorders .
	manualset3
162227	1	412013	7	NULL	NULL	0	NULL	receptive field size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptive field size of nociceptive-specific and wide-dynamic-range neurons in the superficial and deep spinal dorsal horn recorded 24 h after injection of CFA was significantly reduced to 73 + / - 6 % ( P less than 0.05 , n = 8 ) and 74 + / - 4 % ( P less than 0.05 , n = 8 ) of control values , respectively , by a cumulative dose of 3 mg/kg of MK-801 ( i.v. ) .
	manualset3
162228	2	412013	7	NULL	NULL	0	NULL	nociceptive-specific neurons	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptive field size of nociceptive-specific and wide-dynamic-range neurons in the superficial and deep spinal dorsal horn recorded 24 h after injection of CFA was significantly reduced to 73 + / - 6 % ( P less than 0.05 , n = 8 ) and 74 + / - 4 % ( P less than 0.05 , n = 8 ) of control values , respectively , by a cumulative dose of 3 mg/kg of MK-801 ( i.v. ) .
	manualset3
162229	3	412013	7	NULL	NULL	0	NULL	wide-dynamic-range neurons	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptive field size of nociceptive-specific and wide-dynamic-range neurons in the superficial and deep spinal dorsal horn recorded 24 h after injection of CFA was significantly reduced to 73 + / - 6 % ( P less than 0.05 , n = 8 ) and 74 + / - 4 % ( P less than 0.05 , n = 8 ) of control values , respectively , by a cumulative dose of 3 mg/kg of MK-801 ( i.v. ) .
	manualset3
162230	4	412013	7	NULL	NULL	0	NULL	superficial and deep spinal dorsal horn	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptive field size of nociceptive-specific and wide-dynamic-range neurons in the superficial and deep spinal dorsal horn recorded 24 h after injection of CFA was significantly reduced to 73 + / - 6 % ( P less than 0.05 , n = 8 ) and 74 + / - 4 % ( P less than 0.05 , n = 8 ) of control values , respectively , by a cumulative dose of 3 mg/kg of MK-801 ( i.v. ) .
	manualset3
162231	5	412013	7	NULL	NULL	0	NULL	24 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptive field size of nociceptive-specific and wide-dynamic-range neurons in the superficial and deep spinal dorsal horn recorded 24 h after injection of CFA was significantly reduced to 73 + / - 6 % ( P less than 0.05 , n = 8 ) and 74 + / - 4 % ( P less than 0.05 , n = 8 ) of control values , respectively , by a cumulative dose of 3 mg/kg of MK-801 ( i.v. ) .
	manualset3
162232	6	412013	7	NULL	NULL	0	NULL	 injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptive field size of nociceptive-specific and wide-dynamic-range neurons in the superficial and deep spinal dorsal horn recorded 24 h after injection of CFA was significantly reduced to 73 + / - 6 % ( P less than 0.05 , n = 8 ) and 74 + / - 4 % ( P less than 0.05 , n = 8 ) of control values , respectively , by a cumulative dose of 3 mg/kg of MK-801 ( i.v. ) .
	manualset3
162233	7	412013	7	NULL	NULL	0	NULL	CFA	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptive field size of nociceptive-specific and wide-dynamic-range neurons in the superficial and deep spinal dorsal horn recorded 24 h after injection of CFA was significantly reduced to 73 + / - 6 % ( P less than 0.05 , n = 8 ) and 74 + / - 4 % ( P less than 0.05 , n = 8 ) of control values , respectively , by a cumulative dose of 3 mg/kg of MK-801 ( i.v. ) .
	manualset3
162234	8	412013	7	NULL	NULL	0	NULL	73 + / - 6 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptive field size of nociceptive-specific and wide-dynamic-range neurons in the superficial and deep spinal dorsal horn recorded 24 h after injection of CFA was significantly reduced to 73 + / - 6 % ( P less than 0.05 , n = 8 ) and 74 + / - 4 % ( P less than 0.05 , n = 8 ) of control values , respectively , by a cumulative dose of 3 mg/kg of MK-801 ( i.v. ) .
	manualset3
162235	9	412013	7	NULL	NULL	0	NULL	P less than 0.05 , n = 8	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptive field size of nociceptive-specific and wide-dynamic-range neurons in the superficial and deep spinal dorsal horn recorded 24 h after injection of CFA was significantly reduced to 73 + / - 6 % ( P less than 0.05 , n = 8 ) and 74 + / - 4 % ( P less than 0.05 , n = 8 ) of control values , respectively , by a cumulative dose of 3 mg/kg of MK-801 ( i.v. ) .
	manualset3
162236	10	412013	7	NULL	NULL	0	NULL	74 + / - 4 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptive field size of nociceptive-specific and wide-dynamic-range neurons in the superficial and deep spinal dorsal horn recorded 24 h after injection of CFA was significantly reduced to 73 + / - 6 % ( P less than 0.05 , n = 8 ) and 74 + / - 4 % ( P less than 0.05 , n = 8 ) of control values , respectively , by a cumulative dose of 3 mg/kg of MK-801 ( i.v. ) .
	manualset3
162237	11	412013	7	NULL	NULL	0	NULL	P less than 0.05 , n = 8	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptive field size of nociceptive-specific and wide-dynamic-range neurons in the superficial and deep spinal dorsal horn recorded 24 h after injection of CFA was significantly reduced to 73 + / - 6 % ( P less than 0.05 , n = 8 ) and 74 + / - 4 % ( P less than 0.05 , n = 8 ) of control values , respectively , by a cumulative dose of 3 mg/kg of MK-801 ( i.v. ) .
	manualset3
162238	12	412013	7	NULL	NULL	0	NULL	control values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptive field size of nociceptive-specific and wide-dynamic-range neurons in the superficial and deep spinal dorsal horn recorded 24 h after injection of CFA was significantly reduced to 73 + / - 6 % ( P less than 0.05 , n = 8 ) and 74 + / - 4 % ( P less than 0.05 , n = 8 ) of control values , respectively , by a cumulative dose of 3 mg/kg of MK-801 ( i.v. ) .
	manualset3
162239	13	412013	7	NULL	NULL	0	NULL	cumulative dose	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptive field size of nociceptive-specific and wide-dynamic-range neurons in the superficial and deep spinal dorsal horn recorded 24 h after injection of CFA was significantly reduced to 73 + / - 6 % ( P less than 0.05 , n = 8 ) and 74 + / - 4 % ( P less than 0.05 , n = 8 ) of control values , respectively , by a cumulative dose of 3 mg/kg of MK-801 ( i.v. ) .
	manualset3
162240	14	412013	7	NULL	NULL	0	NULL	3 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptive field size of nociceptive-specific and wide-dynamic-range neurons in the superficial and deep spinal dorsal horn recorded 24 h after injection of CFA was significantly reduced to 73 + / - 6 % ( P less than 0.05 , n = 8 ) and 74 + / - 4 % ( P less than 0.05 , n = 8 ) of control values , respectively , by a cumulative dose of 3 mg/kg of MK-801 ( i.v. ) .
	manualset3
162241	15	412013	7	NULL	NULL	0	NULL	MK-801	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptive field size of nociceptive-specific and wide-dynamic-range neurons in the superficial and deep spinal dorsal horn recorded 24 h after injection of CFA was significantly reduced to 73 + / - 6 % ( P less than 0.05 , n = 8 ) and 74 + / - 4 % ( P less than 0.05 , n = 8 ) of control values , respectively , by a cumulative dose of 3 mg/kg of MK-801 ( i.v. ) .
	manualset3
162242	16	412013	7	NULL	NULL	0	NULL	i.v.	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptive field size of nociceptive-specific and wide-dynamic-range neurons in the superficial and deep spinal dorsal horn recorded 24 h after injection of CFA was significantly reduced to 73 + / - 6 % ( P less than 0.05 , n = 8 ) and 74 + / - 4 % ( P less than 0.05 , n = 8 ) of control values , respectively , by a cumulative dose of 3 mg/kg of MK-801 ( i.v. ) .
	manualset3
162243	1	412014	7	NULL	NULL	0	NULL	receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptor could not be detected on BSS platelets but was present on platelets from each of 180 normal subjects .
	manualset3
162244	2	412014	7	NULL	NULL	0	NULL	BSS platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptor could not be detected on BSS platelets but was present on platelets from each of 180 normal subjects .
	manualset3
162245	3	412014	7	NULL	NULL	0	NULL	platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptor could not be detected on BSS platelets but was present on platelets from each of 180 normal subjects .
	manualset3
162246	4	412014	7	NULL	NULL	0	NULL	180 normal subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptor could not be detected on BSS platelets but was present on platelets from each of 180 normal subjects .
	manualset3
162248	1	412015	7	NULL	NULL	0	NULL	 receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptor isolated from a membrane preparation incubated in vitro with ( gamma-32P ) ATP incorporated radiolabel predominantly ( greater than 90 % ) into phosphotyrosine .
	manualset3
162249	2	412015	7	NULL	NULL	0	NULL	membrane preparation	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptor isolated from a membrane preparation incubated in vitro with ( gamma-32P ) ATP incorporated radiolabel predominantly ( greater than 90 % ) into phosphotyrosine .
	manualset3
162250	3	412015	7	NULL	NULL	0	NULL	( gamma-32P ) ATP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptor isolated from a membrane preparation incubated in vitro with ( gamma-32P ) ATP incorporated radiolabel predominantly ( greater than 90 % ) into phosphotyrosine .
	manualset3
162251	4	412015	7	NULL	NULL	0	NULL	radiolabel	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptor isolated from a membrane preparation incubated in vitro with ( gamma-32P ) ATP incorporated radiolabel predominantly ( greater than 90 % ) into phosphotyrosine .
	manualset3
162252	5	412015	7	NULL	NULL	0	NULL	 90 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptor isolated from a membrane preparation incubated in vitro with ( gamma-32P ) ATP incorporated radiolabel predominantly ( greater than 90 % ) into phosphotyrosine .
	manualset3
162253	6	412015	7	NULL	NULL	0	NULL	phosphotyrosine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptor isolated from a membrane preparation incubated in vitro with ( gamma-32P ) ATP incorporated radiolabel predominantly ( greater than 90 % ) into phosphotyrosine .
	manualset3
162254	1	412016	7	NULL	NULL	0	NULL	receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptor was titrated with variable concentrations of ( 3H ) estradiol with or without estriol ; the estriol was maintained in a constant molar ratio to the ( 3H ) estradiol concentration .
	manualset3
162255	2	412016	7	NULL	NULL	0	NULL	variable concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptor was titrated with variable concentrations of ( 3H ) estradiol with or without estriol ; the estriol was maintained in a constant molar ratio to the ( 3H ) estradiol concentration .
	manualset3
162256	3	412016	7	NULL	NULL	0	NULL	( 3H ) estradiol 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptor was titrated with variable concentrations of ( 3H ) estradiol with or without estriol ; the estriol was maintained in a constant molar ratio to the ( 3H ) estradiol concentration .
	manualset3
162257	4	412016	7	NULL	NULL	0	NULL	estriol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptor was titrated with variable concentrations of ( 3H ) estradiol with or without estriol ; the estriol was maintained in a constant molar ratio to the ( 3H ) estradiol concentration .
	manualset3
162258	5	412016	7	NULL	NULL	0	NULL	estriol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptor was titrated with variable concentrations of ( 3H ) estradiol with or without estriol ; the estriol was maintained in a constant molar ratio to the ( 3H ) estradiol concentration .
	manualset3
162259	6	412016	7	NULL	NULL	0	NULL	constant molar ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptor was titrated with variable concentrations of ( 3H ) estradiol with or without estriol ; the estriol was maintained in a constant molar ratio to the ( 3H ) estradiol concentration .
	manualset3
162260	7	412016	7	NULL	NULL	NULL	NULL	( 3H ) estradiol concentration	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The receptor was titrated with variable concentrations of ( 3H ) estradiol with or without estriol ; the estriol was maintained in a constant molar ratio to the ( 3H ) estradiol concentration .
	manualset3
162262	1	412017	7	NULL	NULL	0	NULL	 receptors RAR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptors RAR , and were also detected , each receptor exhibiting differing subcellular locations implying their potential regulation of both transcription and non-genomic actions .
	manualset3
162263	2	412017	7	NULL	NULL	0	NULL	receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptors RAR , and were also detected , each receptor exhibiting differing subcellular locations implying their potential regulation of both transcription and non-genomic actions .
	manualset3
162264	3	412017	7	NULL	NULL	NULL	NULL	subcellular locations 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The receptors RAR , and were also detected , each receptor exhibiting differing subcellular locations implying their potential regulation of both transcription and non-genomic actions .
	manualset3
162265	4	412017	7	NULL	NULL	0	NULL	regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptors RAR , and were also detected , each receptor exhibiting differing subcellular locations implying their potential regulation of both transcription and non-genomic actions .
	manualset3
162266	5	412017	7	NULL	NULL	0	NULL	transcription 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptors RAR , and were also detected , each receptor exhibiting differing subcellular locations implying their potential regulation of both transcription and non-genomic actions .
	manualset3
162267	6	412017	7	NULL	NULL	0	NULL	non-genomic actions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The receptors RAR , and were also detected , each receptor exhibiting differing subcellular locations implying their potential regulation of both transcription and non-genomic actions .
	manualset3
162268	1	412018	7	NULL	NULL	0	NULL	Abnormal microcirculation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Abnormal microcirculation within meninges is common in many neurological diseases .
	manualset3
162269	2	412018	7	NULL	NULL	0	NULL	meninges	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Abnormal microcirculation within meninges is common in many neurological diseases .
	manualset3
162270	3	412018	7	NULL	NULL	0	NULL	neurological diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Abnormal microcirculation within meninges is common in many neurological diseases .
	manualset3
162271	1	412019	7	NULL	NULL	0	NULL	recognition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition and proper designation of BL is important because treatment differs from that of precursor B-cell acute lymphoblastic leukemia ( pre-B ALL ) .
	manualset3
162272	2	412019	7	NULL	NULL	0	NULL	 designation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition and proper designation of BL is important because treatment differs from that of precursor B-cell acute lymphoblastic leukemia ( pre-B ALL ) .
	manualset3
162273	3	412019	7	NULL	NULL	0	NULL	BL	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition and proper designation of BL is important because treatment differs from that of precursor B-cell acute lymphoblastic leukemia ( pre-B ALL ) .
	manualset3
162274	4	412019	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition and proper designation of BL is important because treatment differs from that of precursor B-cell acute lymphoblastic leukemia ( pre-B ALL ) .
	manualset3
162275	5	412019	7	NULL	NULL	NULL	NULL	precursor B-cell acute lymphoblastic leukemia ( pre-B ALL )	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The recognition and proper designation of BL is important because treatment differs from that of precursor B-cell acute lymphoblastic leukemia ( pre-B ALL ) .
	manualset3
162276	1	412020	7	NULL	NULL	NULL	NULL	 recognition	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The recognition of extinct or extant life signatures in the terrestrial geological record is fundamentally dependent upon the understanding of both the structural morphology and chemical composition of relict biomaterials ; the identification of cyanobacterial colonies that have adapted biogeologically their mineral matrices in early evolutionary processes is a fundamental step in the acquisition of analytical data from remote planetary probes designed for life-detection experiments , particularly on Mars and on the planetary satellite moons , Europa and Titan .
	manualset3
162278	2	412020	7	NULL	NULL	NULL	NULL	 life signatures	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The recognition of extinct or extant life signatures in the terrestrial geological record is fundamentally dependent upon the understanding of both the structural morphology and chemical composition of relict biomaterials ; the identification of cyanobacterial colonies that have adapted biogeologically their mineral matrices in early evolutionary processes is a fundamental step in the acquisition of analytical data from remote planetary probes designed for life-detection experiments , particularly on Mars and on the planetary satellite moons , Europa and Titan .
	manualset3
162279	4	412020	7	NULL	NULL	0	NULL	terrestrial geological record	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of extinct or extant life signatures in the terrestrial geological record is fundamentally dependent upon the understanding of both the structural morphology and chemical composition of relict biomaterials ; the identification of cyanobacterial colonies that have adapted biogeologically their mineral matrices in early evolutionary processes is a fundamental step in the acquisition of analytical data from remote planetary probes designed for life-detection experiments , particularly on Mars and on the planetary satellite moons , Europa and Titan .
	manualset3
162280	5	412020	7	NULL	NULL	NULL	NULL	understanding	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The recognition of extinct or extant life signatures in the terrestrial geological record is fundamentally dependent upon the understanding of both the structural morphology and chemical composition of relict biomaterials ; the identification of cyanobacterial colonies that have adapted biogeologically their mineral matrices in early evolutionary processes is a fundamental step in the acquisition of analytical data from remote planetary probes designed for life-detection experiments , particularly on Mars and on the planetary satellite moons , Europa and Titan .
	manualset3
162281	6	412020	7	NULL	NULL	0	NULL	structural morphology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of extinct or extant life signatures in the terrestrial geological record is fundamentally dependent upon the understanding of both the structural morphology and chemical composition of relict biomaterials ; the identification of cyanobacterial colonies that have adapted biogeologically their mineral matrices in early evolutionary processes is a fundamental step in the acquisition of analytical data from remote planetary probes designed for life-detection experiments , particularly on Mars and on the planetary satellite moons , Europa and Titan .
	manualset3
162282	7	412020	7	NULL	NULL	0	NULL	chemical composition 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of extinct or extant life signatures in the terrestrial geological record is fundamentally dependent upon the understanding of both the structural morphology and chemical composition of relict biomaterials ; the identification of cyanobacterial colonies that have adapted biogeologically their mineral matrices in early evolutionary processes is a fundamental step in the acquisition of analytical data from remote planetary probes designed for life-detection experiments , particularly on Mars and on the planetary satellite moons , Europa and Titan .
	manualset3
162283	8	412020	7	NULL	NULL	0	NULL	relict biomaterials	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of extinct or extant life signatures in the terrestrial geological record is fundamentally dependent upon the understanding of both the structural morphology and chemical composition of relict biomaterials ; the identification of cyanobacterial colonies that have adapted biogeologically their mineral matrices in early evolutionary processes is a fundamental step in the acquisition of analytical data from remote planetary probes designed for life-detection experiments , particularly on Mars and on the planetary satellite moons , Europa and Titan .
	manualset3
162284	9	412020	7	NULL	NULL	0	NULL	 identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of extinct or extant life signatures in the terrestrial geological record is fundamentally dependent upon the understanding of both the structural morphology and chemical composition of relict biomaterials ; the identification of cyanobacterial colonies that have adapted biogeologically their mineral matrices in early evolutionary processes is a fundamental step in the acquisition of analytical data from remote planetary probes designed for life-detection experiments , particularly on Mars and on the planetary satellite moons , Europa and Titan .
	manualset3
162285	10	412020	7	NULL	NULL	0	NULL	cyanobacterial colonies 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of extinct or extant life signatures in the terrestrial geological record is fundamentally dependent upon the understanding of both the structural morphology and chemical composition of relict biomaterials ; the identification of cyanobacterial colonies that have adapted biogeologically their mineral matrices in early evolutionary processes is a fundamental step in the acquisition of analytical data from remote planetary probes designed for life-detection experiments , particularly on Mars and on the planetary satellite moons , Europa and Titan .
	manualset3
162286	11	412020	7	NULL	NULL	0	NULL	mineral matrices	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of extinct or extant life signatures in the terrestrial geological record is fundamentally dependent upon the understanding of both the structural morphology and chemical composition of relict biomaterials ; the identification of cyanobacterial colonies that have adapted biogeologically their mineral matrices in early evolutionary processes is a fundamental step in the acquisition of analytical data from remote planetary probes designed for life-detection experiments , particularly on Mars and on the planetary satellite moons , Europa and Titan .
	manualset3
162287	12	412020	7	NULL	NULL	0	NULL	 early evolutionary processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of extinct or extant life signatures in the terrestrial geological record is fundamentally dependent upon the understanding of both the structural morphology and chemical composition of relict biomaterials ; the identification of cyanobacterial colonies that have adapted biogeologically their mineral matrices in early evolutionary processes is a fundamental step in the acquisition of analytical data from remote planetary probes designed for life-detection experiments , particularly on Mars and on the planetary satellite moons , Europa and Titan .
	manualset3
162288	13	412020	7	NULL	NULL	0	NULL	fundamental step	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of extinct or extant life signatures in the terrestrial geological record is fundamentally dependent upon the understanding of both the structural morphology and chemical composition of relict biomaterials ; the identification of cyanobacterial colonies that have adapted biogeologically their mineral matrices in early evolutionary processes is a fundamental step in the acquisition of analytical data from remote planetary probes designed for life-detection experiments , particularly on Mars and on the planetary satellite moons , Europa and Titan .
	manualset3
162289	14	412020	7	NULL	NULL	0	NULL	acquisition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of extinct or extant life signatures in the terrestrial geological record is fundamentally dependent upon the understanding of both the structural morphology and chemical composition of relict biomaterials ; the identification of cyanobacterial colonies that have adapted biogeologically their mineral matrices in early evolutionary processes is a fundamental step in the acquisition of analytical data from remote planetary probes designed for life-detection experiments , particularly on Mars and on the planetary satellite moons , Europa and Titan .
	manualset3
162290	15	412020	7	NULL	NULL	0	NULL	analytical data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of extinct or extant life signatures in the terrestrial geological record is fundamentally dependent upon the understanding of both the structural morphology and chemical composition of relict biomaterials ; the identification of cyanobacterial colonies that have adapted biogeologically their mineral matrices in early evolutionary processes is a fundamental step in the acquisition of analytical data from remote planetary probes designed for life-detection experiments , particularly on Mars and on the planetary satellite moons , Europa and Titan .
	manualset3
162291	16	412020	7	NULL	NULL	0	NULL	remote planetary probes	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of extinct or extant life signatures in the terrestrial geological record is fundamentally dependent upon the understanding of both the structural morphology and chemical composition of relict biomaterials ; the identification of cyanobacterial colonies that have adapted biogeologically their mineral matrices in early evolutionary processes is a fundamental step in the acquisition of analytical data from remote planetary probes designed for life-detection experiments , particularly on Mars and on the planetary satellite moons , Europa and Titan .
	manualset3
162292	17	412020	7	NULL	NULL	0	NULL	life-detection experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of extinct or extant life signatures in the terrestrial geological record is fundamentally dependent upon the understanding of both the structural morphology and chemical composition of relict biomaterials ; the identification of cyanobacterial colonies that have adapted biogeologically their mineral matrices in early evolutionary processes is a fundamental step in the acquisition of analytical data from remote planetary probes designed for life-detection experiments , particularly on Mars and on the planetary satellite moons , Europa and Titan .
	manualset3
162293	18	412020	7	NULL	NULL	NULL	NULL	 Mars	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The recognition of extinct or extant life signatures in the terrestrial geological record is fundamentally dependent upon the understanding of both the structural morphology and chemical composition of relict biomaterials ; the identification of cyanobacterial colonies that have adapted biogeologically their mineral matrices in early evolutionary processes is a fundamental step in the acquisition of analytical data from remote planetary probes designed for life-detection experiments , particularly on Mars and on the planetary satellite moons , Europa and Titan .
	manualset3
162294	19	412020	7	NULL	NULL	NULL	NULL	 planetary satellite moons	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The recognition of extinct or extant life signatures in the terrestrial geological record is fundamentally dependent upon the understanding of both the structural morphology and chemical composition of relict biomaterials ; the identification of cyanobacterial colonies that have adapted biogeologically their mineral matrices in early evolutionary processes is a fundamental step in the acquisition of analytical data from remote planetary probes designed for life-detection experiments , particularly on Mars and on the planetary satellite moons , Europa and Titan .
	manualset3
162295	20	412020	7	NULL	NULL	NULL	NULL	Europa	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The recognition of extinct or extant life signatures in the terrestrial geological record is fundamentally dependent upon the understanding of both the structural morphology and chemical composition of relict biomaterials ; the identification of cyanobacterial colonies that have adapted biogeologically their mineral matrices in early evolutionary processes is a fundamental step in the acquisition of analytical data from remote planetary probes designed for life-detection experiments , particularly on Mars and on the planetary satellite moons , Europa and Titan .
	manualset3
162296	21	412020	7	NULL	NULL	NULL	NULL	Titan 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The recognition of extinct or extant life signatures in the terrestrial geological record is fundamentally dependent upon the understanding of both the structural morphology and chemical composition of relict biomaterials ; the identification of cyanobacterial colonies that have adapted biogeologically their mineral matrices in early evolutionary processes is a fundamental step in the acquisition of analytical data from remote planetary probes designed for life-detection experiments , particularly on Mars and on the planetary satellite moons , Europa and Titan .
	manualset3
162297	1	412021	7	NULL	NULL	0	NULL	 recognition 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of low amounts of DMPK-1 and DMPK-2 indicates the high affinity of these antibodies .
	manualset3
162298	2	412021	7	NULL	NULL	0	NULL	low amounts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of low amounts of DMPK-1 and DMPK-2 indicates the high affinity of these antibodies .
	manualset3
162299	3	412021	7	NULL	NULL	0	NULL	DMPK-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of low amounts of DMPK-1 and DMPK-2 indicates the high affinity of these antibodies .
	manualset3
162300	4	412021	7	NULL	NULL	0	NULL	DMPK-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of low amounts of DMPK-1 and DMPK-2 indicates the high affinity of these antibodies .
	manualset3
162301	5	412021	7	NULL	NULL	0	NULL	high affinity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of low amounts of DMPK-1 and DMPK-2 indicates the high affinity of these antibodies .
	manualset3
162302	6	412021	7	NULL	NULL	0	NULL	antibodies	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of low amounts of DMPK-1 and DMPK-2 indicates the high affinity of these antibodies .
	manualset3
162303	1	412022	7	NULL	NULL	0	NULL	recognition 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of the adults ' responsibility ( especially choice of partners , functionalization of the child to facilitate the separation from the own parents , to maintain the image of an intact family or the struggle for power at the cost of the children ) diminishes the feelings of guilt of the children .
	manualset3
162304	2	412022	7	NULL	NULL	0	NULL	adults ' responsibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of the adults ' responsibility ( especially choice of partners , functionalization of the child to facilitate the separation from the own parents , to maintain the image of an intact family or the struggle for power at the cost of the children ) diminishes the feelings of guilt of the children .
	manualset3
162305	3	412022	7	NULL	NULL	NULL	NULL	partners	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The recognition of the adults ' responsibility ( especially choice of partners , functionalization of the child to facilitate the separation from the own parents , to maintain the image of an intact family or the struggle for power at the cost of the children ) diminishes the feelings of guilt of the children .
	manualset3
162306	4	412022	7	NULL	NULL	0	NULL	functionalization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of the adults ' responsibility ( especially choice of partners , functionalization of the child to facilitate the separation from the own parents , to maintain the image of an intact family or the struggle for power at the cost of the children ) diminishes the feelings of guilt of the children .
	manualset3
162307	5	412022	7	NULL	NULL	0	NULL	child	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of the adults ' responsibility ( especially choice of partners , functionalization of the child to facilitate the separation from the own parents , to maintain the image of an intact family or the struggle for power at the cost of the children ) diminishes the feelings of guilt of the children .
	manualset3
162308	6	412022	7	NULL	NULL	0	NULL	 separation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of the adults ' responsibility ( especially choice of partners , functionalization of the child to facilitate the separation from the own parents , to maintain the image of an intact family or the struggle for power at the cost of the children ) diminishes the feelings of guilt of the children .
	manualset3
162309	7	412022	7	NULL	NULL	0	NULL	 parents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of the adults ' responsibility ( especially choice of partners , functionalization of the child to facilitate the separation from the own parents , to maintain the image of an intact family or the struggle for power at the cost of the children ) diminishes the feelings of guilt of the children .
	manualset3
162310	8	412022	7	NULL	NULL	0	NULL	image	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of the adults ' responsibility ( especially choice of partners , functionalization of the child to facilitate the separation from the own parents , to maintain the image of an intact family or the struggle for power at the cost of the children ) diminishes the feelings of guilt of the children .
	manualset3
162311	9	412022	7	NULL	NULL	0	NULL	intact family	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of the adults ' responsibility ( especially choice of partners , functionalization of the child to facilitate the separation from the own parents , to maintain the image of an intact family or the struggle for power at the cost of the children ) diminishes the feelings of guilt of the children .
	manualset3
162312	10	412022	7	NULL	NULL	0	NULL	 power	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of the adults ' responsibility ( especially choice of partners , functionalization of the child to facilitate the separation from the own parents , to maintain the image of an intact family or the struggle for power at the cost of the children ) diminishes the feelings of guilt of the children .
	manualset3
162313	11	412022	7	NULL	NULL	NULL	NULL	 cost	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The recognition of the adults ' responsibility ( especially choice of partners , functionalization of the child to facilitate the separation from the own parents , to maintain the image of an intact family or the struggle for power at the cost of the children ) diminishes the feelings of guilt of the children .
	manualset3
162314	12	412022	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of the adults ' responsibility ( especially choice of partners , functionalization of the child to facilitate the separation from the own parents , to maintain the image of an intact family or the struggle for power at the cost of the children ) diminishes the feelings of guilt of the children .
	manualset3
162315	13	412022	7	NULL	NULL	NULL	NULL	feelings	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The recognition of the adults ' responsibility ( especially choice of partners , functionalization of the child to facilitate the separation from the own parents , to maintain the image of an intact family or the struggle for power at the cost of the children ) diminishes the feelings of guilt of the children .
	manualset3
162316	14	412022	7	NULL	NULL	NULL	NULL	guilt 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The recognition of the adults ' responsibility ( especially choice of partners , functionalization of the child to facilitate the separation from the own parents , to maintain the image of an intact family or the struggle for power at the cost of the children ) diminishes the feelings of guilt of the children .
	manualset3
162317	15	412022	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of the adults ' responsibility ( especially choice of partners , functionalization of the child to facilitate the separation from the own parents , to maintain the image of an intact family or the struggle for power at the cost of the children ) diminishes the feelings of guilt of the children .
	manualset3
162324	16	412022	7	NULL	NULL	0	NULL	struggle	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition of the adults ' responsibility ( especially choice of partners , functionalization of the child to facilitate the separation from the own parents , to maintain the image of an intact family or the struggle for power at the cost of the children ) diminishes the feelings of guilt of the children .
	manualset3
162318	1	412023	7	NULL	NULL	0	NULL	recognition potential ( RP )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition potential ( RP ) was distinguished from P3 and eye blink responses by its sensitivity to visual area stimulated .
	manualset3
162320	2	412023	7	NULL	NULL	0	NULL	P3 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition potential ( RP ) was distinguished from P3 and eye blink responses by its sensitivity to visual area stimulated .
	manualset3
162321	3	412023	7	NULL	NULL	0	NULL	eye blink responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition potential ( RP ) was distinguished from P3 and eye blink responses by its sensitivity to visual area stimulated .
	manualset3
162322	4	412023	7	NULL	NULL	0	NULL	sensitivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition potential ( RP ) was distinguished from P3 and eye blink responses by its sensitivity to visual area stimulated .
	manualset3
162323	5	412023	7	NULL	NULL	0	NULL	visual area	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The recognition potential ( RP ) was distinguished from P3 and eye blink responses by its sensitivity to visual area stimulated .
	manualset3
162325	1	412024	7	NULL	NULL	0	NULL	recombinant A1 adhesin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The recombinant A1 adhesin therefore has potential in the development of a P. gingivalis vaccine .
	manualset3
162326	2	412024	7	NULL	NULL	NULL	NULL	potential	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The recombinant A1 adhesin therefore has potential in the development of a P. gingivalis vaccine .
	manualset3
162327	3	412024	7	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The recombinant A1 adhesin therefore has potential in the development of a P. gingivalis vaccine .
	manualset3
162328	4	412024	7	NULL	NULL	0	NULL	P. gingivalis vaccine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The recombinant A1 adhesin therefore has potential in the development of a P. gingivalis vaccine .
	manualset3
162329	1	412025	7	NULL	NULL	0	NULL	recombinant TcRAB5 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The recombinant TcRAB5 protein was able to bind and hydrolyze GTP .
	manualset3
162330	2	412025	7	NULL	NULL	0	NULL	 GTP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The recombinant TcRAB5 protein was able to bind and hydrolyze GTP .
	manualset3
162331	1	412026	7	NULL	NULL	0	NULL	recombinant acocostatin peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The recombinant acocostatin peptide was produced and purified as GST-fusion .
	manualset3
162332	2	412026	7	NULL	NULL	0	NULL	GST-fusion	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The recombinant acocostatin peptide was produced and purified as GST-fusion .
	manualset3
162333	1	412027	7	NULL	NULL	0	NULL	recombinant enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The recombinant enzyme exhibited high thermal activity and thermostability with optimal activity between pH 6.5 and 7.0 .
	manualset3
162334	2	412027	7	NULL	NULL	0	NULL	high thermal activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The recombinant enzyme exhibited high thermal activity and thermostability with optimal activity between pH 6.5 and 7.0 .
	manualset3
162335	3	412027	7	NULL	NULL	0	NULL	thermostability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The recombinant enzyme exhibited high thermal activity and thermostability with optimal activity between pH 6.5 and 7.0 .
	manualset3
162336	4	412027	7	NULL	NULL	0	NULL	optimal activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The recombinant enzyme exhibited high thermal activity and thermostability with optimal activity between pH 6.5 and 7.0 .
	manualset3
162337	5	412027	7	NULL	NULL	0	NULL	pH 6.5	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The recombinant enzyme exhibited high thermal activity and thermostability with optimal activity between pH 6.5 and 7.0 .
	manualset3
162338	6	412027	7	NULL	NULL	0	NULL	pH 7.0	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The recombinant enzyme exhibited high thermal activity and thermostability with optimal activity between pH 6.5 and 7.0 .
	manualset3
162339	1	412028	7	NULL	NULL	0	NULL	Abnormal molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Abnormal molecules could form disulfide bond between the A alpha Cys16 residues .
	manualset3
162340	2	412028	7	NULL	NULL	0	NULL	disulfide bond 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Abnormal molecules could form disulfide bond between the A alpha Cys16 residues .
	manualset3
162341	3	412028	7	NULL	NULL	0	NULL	A alpha Cys16 residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Abnormal molecules could form disulfide bond between the A alpha Cys16 residues .
	manualset3
162342	1	412029	7	NULL	NULL	0	NULL	recombinant polypeptide , BPI '	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The recombinant polypeptide , BPI ' , was solubilized and conditions under which it folded to give the active protein were determined .
	manualset3
162343	2	412029	7	NULL	NULL	0	NULL	conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The recombinant polypeptide , BPI ' , was solubilized and conditions under which it folded to give the active protein were determined .
	manualset3
162344	3	412029	7	NULL	NULL	0	NULL	active protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The recombinant polypeptide , BPI ' , was solubilized and conditions under which it folded to give the active protein were determined .
	manualset3
162345	1	412030	7	NULL	NULL	0	NULL	recombinant rat OSC 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The recombinant rat OSC expressed was efficiently labeled by the mechanism-based inhibitor ( 3H ) 29-MOS .
	manualset3
162346	2	412030	7	NULL	NULL	NULL	NULL	mechanism-based inhibitor ( 3H ) 29-MOS	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The recombinant rat OSC expressed was efficiently labeled by the mechanism-based inhibitor ( 3H ) 29-MOS .
	manualset3
162363	1	412031	7	NULL	NULL	0	NULL	recombinants	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The recombinants generated with this fragment were at least 50-fold more neuroviurlent than RE6 , as determined by the plaque forming unit to lethal dose 50 % assay .
	manualset3
162364	2	412031	7	NULL	NULL	0	NULL	fragment	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The recombinants generated with this fragment were at least 50-fold more neuroviurlent than RE6 , as determined by the plaque forming unit to lethal dose 50 % assay .
	manualset3
162365	3	412031	7	NULL	NULL	0	NULL	50-fold 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The recombinants generated with this fragment were at least 50-fold more neuroviurlent than RE6 , as determined by the plaque forming unit to lethal dose 50 % assay .
	manualset3
162366	4	412031	7	NULL	NULL	0	NULL	 neuroviurlent	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The recombinants generated with this fragment were at least 50-fold more neuroviurlent than RE6 , as determined by the plaque forming unit to lethal dose 50 % assay .
	manualset3
162367	5	412031	7	NULL	NULL	0	NULL	RE6	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The recombinants generated with this fragment were at least 50-fold more neuroviurlent than RE6 , as determined by the plaque forming unit to lethal dose 50 % assay .
	manualset3
162368	6	412031	7	NULL	NULL	0	NULL	 plaque forming unit	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The recombinants generated with this fragment were at least 50-fold more neuroviurlent than RE6 , as determined by the plaque forming unit to lethal dose 50 % assay .
	manualset3
162369	7	412031	7	NULL	NULL	0	NULL	lethal dose 50 % assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The recombinants generated with this fragment were at least 50-fold more neuroviurlent than RE6 , as determined by the plaque forming unit to lethal dose 50 % assay .
	manualset3
162370	1	412032	7	NULL	NULL	0	NULL	 role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The recommended role of ultraviolet germicidal irradiation ( UVGI ) is to reduce the risk of tuberculosis ( TB ) transmission in health care facilities .
	manualset3
162371	2	412032	7	NULL	NULL	0	NULL	ultraviolet germicidal irradiation ( UVGI )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The recommended role of ultraviolet germicidal irradiation ( UVGI ) is to reduce the risk of tuberculosis ( TB ) transmission in health care facilities .
	manualset3
162372	3	412032	7	NULL	NULL	0	NULL	risk 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The recommended role of ultraviolet germicidal irradiation ( UVGI ) is to reduce the risk of tuberculosis ( TB ) transmission in health care facilities .
	manualset3
162373	4	412032	7	NULL	NULL	0	NULL	tuberculosis ( TB ) transmission	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The recommended role of ultraviolet germicidal irradiation ( UVGI ) is to reduce the risk of tuberculosis ( TB ) transmission in health care facilities .
	manualset3
162374	5	412032	7	NULL	NULL	0	NULL	health care facilities	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The recommended role of ultraviolet germicidal irradiation ( UVGI ) is to reduce the risk of tuberculosis ( TB ) transmission in health care facilities .
	manualset3
162375	1	412033	7	NULL	NULL	NULL	NULL	 parasite fauna	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The recorded parasite fauna is represented by marine , brackish water , and probably also freshwater components .
	manualset3
162376	2	412033	7	NULL	NULL	0	NULL	 marine water	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The recorded parasite fauna is represented by marine , brackish water , and probably also freshwater components .
	manualset3
162377	3	412033	7	NULL	NULL	0	NULL	 brackish water	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The recorded parasite fauna is represented by marine , brackish water , and probably also freshwater components .
	manualset3
162378	4	412033	7	NULL	NULL	0	NULL	freshwater components	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The recorded parasite fauna is represented by marine , brackish water , and probably also freshwater components .
	manualset3
162379	1	412034	7	NULL	NULL	0	NULL	records	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The records were reviewed to identify comparative and randomized controlled trials evaluating the effect of screening on prostate cancer .
	manualset3
162380	2	412034	7	NULL	NULL	0	NULL	comparative and randomized controlled trials	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The records were reviewed to identify comparative and randomized controlled trials evaluating the effect of screening on prostate cancer .
	manualset3
162381	3	412034	7	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The records were reviewed to identify comparative and randomized controlled trials evaluating the effect of screening on prostate cancer .
	manualset3
162382	4	412034	7	NULL	NULL	0	NULL	screening	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The records were reviewed to identify comparative and randomized controlled trials evaluating the effect of screening on prostate cancer .
	manualset3
162383	5	412034	7	NULL	NULL	NULL	NULL	prostate cancer	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The records were reviewed to identify comparative and randomized controlled trials evaluating the effect of screening on prostate cancer .
	manualset3
162384	1	412035	7	NULL	NULL	NULL	NULL	 redox stress	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The redox stress hypothesis of aging .
	manualset3
162385	2	412035	7	NULL	NULL	0	NULL	hypothesis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The redox stress hypothesis of aging .
	manualset3
162386	3	412035	7	NULL	NULL	0	NULL	aging	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The redox stress hypothesis of aging .
	manualset3
162387	1	412036	7	NULL	NULL	0	NULL	reduced cytochrome b	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduced cytochrome b in the enzyme complex could be oxidized by CoM-S-S-HTP and re-reduced by H2 .
	manualset3
162388	2	412036	7	NULL	NULL	0	NULL	enzyme complex	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduced cytochrome b in the enzyme complex could be oxidized by CoM-S-S-HTP and re-reduced by H2 .
	manualset3
162389	3	412036	7	NULL	NULL	0	NULL	CoM-S-S-HTP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduced cytochrome b in the enzyme complex could be oxidized by CoM-S-S-HTP and re-reduced by H2 .
	manualset3
162390	4	412036	7	NULL	NULL	0	NULL	H2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduced cytochrome b in the enzyme complex could be oxidized by CoM-S-S-HTP and re-reduced by H2 .
	manualset3
162391	1	412037	7	NULL	NULL	NULL	NULL	Abnormal structure	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Abnormal structure and dysfunction of tumor blood vessels are responsible for these conditions .
	manualset3
162392	2	412037	7	NULL	NULL	NULL	NULL	dysfunction	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Abnormal structure and dysfunction of tumor blood vessels are responsible for these conditions .
	manualset3
162393	3	412037	7	NULL	NULL	NULL	NULL	tumor blood vessels	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Abnormal structure and dysfunction of tumor blood vessels are responsible for these conditions .
	manualset3
162394	4	412037	7	NULL	NULL	NULL	NULL	conditions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Abnormal structure and dysfunction of tumor blood vessels are responsible for these conditions .
	manualset3
162395	1	412038	7	NULL	NULL	NULL	NULL	reduced expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reduced expression of Fas in corresponding cancer cells in combination with the ability to express FasL might facilitate immune escape .
	manualset3
162396	2	412038	7	NULL	NULL	0	NULL	Fas	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduced expression of Fas in corresponding cancer cells in combination with the ability to express FasL might facilitate immune escape .
	manualset3
162397	3	412038	7	NULL	NULL	0	NULL	cancer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduced expression of Fas in corresponding cancer cells in combination with the ability to express FasL might facilitate immune escape .
	manualset3
162398	4	412038	7	NULL	NULL	NULL	NULL	combination	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reduced expression of Fas in corresponding cancer cells in combination with the ability to express FasL might facilitate immune escape .
	manualset3
162399	5	412038	7	NULL	NULL	NULL	NULL	ability	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reduced expression of Fas in corresponding cancer cells in combination with the ability to express FasL might facilitate immune escape .
	manualset3
162400	6	412038	7	NULL	NULL	0	NULL	FasL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduced expression of Fas in corresponding cancer cells in combination with the ability to express FasL might facilitate immune escape .
	manualset3
162401	7	412038	7	NULL	NULL	0	NULL	immune escape	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduced expression of Fas in corresponding cancer cells in combination with the ability to express FasL might facilitate immune escape .
	manualset3
162402	1	412039	7	NULL	NULL	NULL	NULL	reduction	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reduction by nitric oxide donors of Ca2 + mobilization in stimulated platelets lead us to investigate the direct effect of authentic NO on ATP-dependent Ca2 + uptake into platelet membrane vesicles .
	manualset3
162403	2	412039	7	NULL	NULL	0	NULL	nitric oxide donors 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction by nitric oxide donors of Ca2 + mobilization in stimulated platelets lead us to investigate the direct effect of authentic NO on ATP-dependent Ca2 + uptake into platelet membrane vesicles .
	manualset3
162404	3	412039	7	NULL	NULL	NULL	NULL	Ca2 + mobilization	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reduction by nitric oxide donors of Ca2 + mobilization in stimulated platelets lead us to investigate the direct effect of authentic NO on ATP-dependent Ca2 + uptake into platelet membrane vesicles .
	manualset3
162405	4	412039	7	NULL	NULL	0	NULL	stimulated platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction by nitric oxide donors of Ca2 + mobilization in stimulated platelets lead us to investigate the direct effect of authentic NO on ATP-dependent Ca2 + uptake into platelet membrane vesicles .
	manualset3
162406	5	412039	7	NULL	NULL	NULL	NULL	direct effect	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reduction by nitric oxide donors of Ca2 + mobilization in stimulated platelets lead us to investigate the direct effect of authentic NO on ATP-dependent Ca2 + uptake into platelet membrane vesicles .
	manualset3
162407	6	412039	7	NULL	NULL	0	NULL	authentic NO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction by nitric oxide donors of Ca2 + mobilization in stimulated platelets lead us to investigate the direct effect of authentic NO on ATP-dependent Ca2 + uptake into platelet membrane vesicles .
	manualset3
162408	7	412039	7	NULL	NULL	NULL	NULL	ATP-dependent Ca2 + uptake	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reduction by nitric oxide donors of Ca2 + mobilization in stimulated platelets lead us to investigate the direct effect of authentic NO on ATP-dependent Ca2 + uptake into platelet membrane vesicles .
	manualset3
162409	8	412039	7	NULL	NULL	0	NULL	platelet membrane vesicles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction by nitric oxide donors of Ca2 + mobilization in stimulated platelets lead us to investigate the direct effect of authentic NO on ATP-dependent Ca2 + uptake into platelet membrane vesicles .
	manualset3
162410	1	412040	7	NULL	NULL	NULL	NULL	reduction	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reduction of ERRgamma may have two possible sequelae : disarrangement of vaginal development and high risk of vaginal cancer .
	manualset3
162411	2	412040	7	NULL	NULL	0	NULL	ERRgamma	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of ERRgamma may have two possible sequelae : disarrangement of vaginal development and high risk of vaginal cancer .
	manualset3
162412	3	412040	7	NULL	NULL	0	NULL	disarrangement	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of ERRgamma may have two possible sequelae : disarrangement of vaginal development and high risk of vaginal cancer .
	manualset3
162413	4	412040	7	NULL	NULL	0	NULL	vaginal development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of ERRgamma may have two possible sequelae : disarrangement of vaginal development and high risk of vaginal cancer .
	manualset3
162414	5	412040	7	NULL	NULL	NULL	NULL	high risk	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reduction of ERRgamma may have two possible sequelae : disarrangement of vaginal development and high risk of vaginal cancer .
	manualset3
162415	6	412040	7	NULL	NULL	0	NULL	vaginal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of ERRgamma may have two possible sequelae : disarrangement of vaginal development and high risk of vaginal cancer .
	manualset3
163799	7	412040	7	NULL	NULL	0	NULL	 two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of ERRgamma may have two possible sequelae : disarrangement of vaginal development and high risk of vaginal cancer .
	manualset3
163800	8	412040	7	NULL	NULL	0	NULL	sequelae	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of ERRgamma may have two possible sequelae : disarrangement of vaginal development and high risk of vaginal cancer .
	manualset3
162416	1	412041	7	NULL	NULL	0	NULL	 reduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of responses to the mixed receptor agonists L-glutamate and L-aspartate may be the result of opposite actions of the catecholamines on the activation of specific excitatory receptors by the amino acids .
	manualset3
162417	2	412041	7	NULL	NULL	0	NULL	responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of responses to the mixed receptor agonists L-glutamate and L-aspartate may be the result of opposite actions of the catecholamines on the activation of specific excitatory receptors by the amino acids .
	manualset3
162418	3	412041	7	NULL	NULL	0	NULL	mixed receptor agonists	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of responses to the mixed receptor agonists L-glutamate and L-aspartate may be the result of opposite actions of the catecholamines on the activation of specific excitatory receptors by the amino acids .
	manualset3
162419	4	412041	7	NULL	NULL	0	NULL	L-glutamate	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of responses to the mixed receptor agonists L-glutamate and L-aspartate may be the result of opposite actions of the catecholamines on the activation of specific excitatory receptors by the amino acids .
	manualset3
162420	5	412041	7	NULL	NULL	0	NULL	L-aspartate	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of responses to the mixed receptor agonists L-glutamate and L-aspartate may be the result of opposite actions of the catecholamines on the activation of specific excitatory receptors by the amino acids .
	manualset3
162421	6	412041	7	NULL	NULL	NULL	NULL	result	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reduction of responses to the mixed receptor agonists L-glutamate and L-aspartate may be the result of opposite actions of the catecholamines on the activation of specific excitatory receptors by the amino acids .
	manualset3
162422	7	412041	7	NULL	NULL	0	NULL	opposite actions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of responses to the mixed receptor agonists L-glutamate and L-aspartate may be the result of opposite actions of the catecholamines on the activation of specific excitatory receptors by the amino acids .
	manualset3
162423	8	412041	7	NULL	NULL	0	NULL	catecholamines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of responses to the mixed receptor agonists L-glutamate and L-aspartate may be the result of opposite actions of the catecholamines on the activation of specific excitatory receptors by the amino acids .
	manualset3
162424	9	412041	7	NULL	NULL	0	NULL	 activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of responses to the mixed receptor agonists L-glutamate and L-aspartate may be the result of opposite actions of the catecholamines on the activation of specific excitatory receptors by the amino acids .
	manualset3
162425	10	412041	7	NULL	NULL	0	NULL	excitatory receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of responses to the mixed receptor agonists L-glutamate and L-aspartate may be the result of opposite actions of the catecholamines on the activation of specific excitatory receptors by the amino acids .
	manualset3
162426	11	412041	7	NULL	NULL	0	NULL	amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of responses to the mixed receptor agonists L-glutamate and L-aspartate may be the result of opposite actions of the catecholamines on the activation of specific excitatory receptors by the amino acids .
	manualset3
162427	1	412042	7	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of stress , perceived risk and discomfort following educational efforts have been supported in past research .
	manualset3
162428	2	412042	7	NULL	NULL	NULL	NULL	stress	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reduction of stress , perceived risk and discomfort following educational efforts have been supported in past research .
	manualset3
162429	3	412042	7	NULL	NULL	NULL	NULL	perceived risk	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reduction of stress , perceived risk and discomfort following educational efforts have been supported in past research .
	manualset3
162430	4	412042	7	NULL	NULL	0	NULL	discomfort 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of stress , perceived risk and discomfort following educational efforts have been supported in past research .
	manualset3
162431	5	412042	7	NULL	NULL	0	NULL	educational efforts 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of stress , perceived risk and discomfort following educational efforts have been supported in past research .
	manualset3
162432	6	412042	7	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of stress , perceived risk and discomfort following educational efforts have been supported in past research .
	manualset3
162433	1	412043	7	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of the bioleaching period and improvement of metals extraction yield will likely allow the practical application of the bioleaching technology for heavy metals removal from fly ash .
	manualset3
162434	2	412043	7	NULL	NULL	0	NULL	 bioleaching period	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of the bioleaching period and improvement of metals extraction yield will likely allow the practical application of the bioleaching technology for heavy metals removal from fly ash .
	manualset3
162435	3	412043	7	NULL	NULL	0	NULL	improvement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of the bioleaching period and improvement of metals extraction yield will likely allow the practical application of the bioleaching technology for heavy metals removal from fly ash .
	manualset3
162436	4	412043	7	NULL	NULL	0	NULL	metals extraction yield	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of the bioleaching period and improvement of metals extraction yield will likely allow the practical application of the bioleaching technology for heavy metals removal from fly ash .
	manualset3
162437	5	412043	7	NULL	NULL	0	NULL	practical application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of the bioleaching period and improvement of metals extraction yield will likely allow the practical application of the bioleaching technology for heavy metals removal from fly ash .
	manualset3
162438	6	412043	7	NULL	NULL	0	NULL	bioleaching technology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of the bioleaching period and improvement of metals extraction yield will likely allow the practical application of the bioleaching technology for heavy metals removal from fly ash .
	manualset3
162439	7	412043	7	NULL	NULL	0	NULL	heavy metals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of the bioleaching period and improvement of metals extraction yield will likely allow the practical application of the bioleaching technology for heavy metals removal from fly ash .
	manualset3
162440	8	412043	7	NULL	NULL	0	NULL	removal 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of the bioleaching period and improvement of metals extraction yield will likely allow the practical application of the bioleaching technology for heavy metals removal from fly ash .
	manualset3
162441	9	412043	7	NULL	NULL	0	NULL	fly ash	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of the bioleaching period and improvement of metals extraction yield will likely allow the practical application of the bioleaching technology for heavy metals removal from fly ash .
	manualset3
162442	1	412044	7	NULL	NULL	0	NULL	 reduction potential 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction potential of the ( FADH - / FADH * ) couple in DNA photolyase was measured , and the value was found to be significantly higher than the values estimated in the literature .
	manualset3
162443	2	412044	7	NULL	NULL	0	NULL	( FADH - / FADH * ) couple 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction potential of the ( FADH - / FADH * ) couple in DNA photolyase was measured , and the value was found to be significantly higher than the values estimated in the literature .
	manualset3
162444	3	412044	7	NULL	NULL	0	NULL	DNA photolyase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction potential of the ( FADH - / FADH * ) couple in DNA photolyase was measured , and the value was found to be significantly higher than the values estimated in the literature .
	manualset3
162445	4	412044	7	NULL	NULL	0	NULL	value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction potential of the ( FADH - / FADH * ) couple in DNA photolyase was measured , and the value was found to be significantly higher than the values estimated in the literature .
	manualset3
162446	5	412044	7	NULL	NULL	0	NULL	values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction potential of the ( FADH - / FADH * ) couple in DNA photolyase was measured , and the value was found to be significantly higher than the values estimated in the literature .
	manualset3
162447	6	412044	7	NULL	NULL	0	NULL	 literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction potential of the ( FADH - / FADH * ) couple in DNA photolyase was measured , and the value was found to be significantly higher than the values estimated in the literature .
	manualset3
162448	1	412045	7	NULL	NULL	0	NULL	 reduction potentials	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction potentials E ( 1/2 ) ( red ) cover a large range of -2.11 V for 2 , 5-diphenyl-1 , 3 , 4 - oxadiazole to -0.76 V for 1 , 2 , 3 , 4 , 5 , 6-hexa ( 5-phenyl-1 , 3 , 4 - oxadiazo-2-yl ) benzene .
	manualset3
162449	2	412045	7	NULL	NULL	0	NULL	E ( 1/2 ) ( red )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction potentials E ( 1/2 ) ( red ) cover a large range of -2.11 V for 2 , 5-diphenyl-1 , 3 , 4 - oxadiazole to -0.76 V for 1 , 2 , 3 , 4 , 5 , 6-hexa ( 5-phenyl-1 , 3 , 4 - oxadiazo-2-yl ) benzene .
	manualset3
162450	3	412045	7	NULL	NULL	0	NULL	-2.11 V	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction potentials E ( 1/2 ) ( red ) cover a large range of -2.11 V for 2 , 5-diphenyl-1 , 3 , 4 - oxadiazole to -0.76 V for 1 , 2 , 3 , 4 , 5 , 6-hexa ( 5-phenyl-1 , 3 , 4 - oxadiazo-2-yl ) benzene .
	manualset3
162451	4	412045	7	NULL	NULL	0	NULL	 2 , 5-diphenyl-1 , 3 , 4 - oxadiazole	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction potentials E ( 1/2 ) ( red ) cover a large range of -2.11 V for 2 , 5-diphenyl-1 , 3 , 4 - oxadiazole to -0.76 V for 1 , 2 , 3 , 4 , 5 , 6-hexa ( 5-phenyl-1 , 3 , 4 - oxadiazo-2-yl ) benzene .
	manualset3
162452	5	412045	7	NULL	NULL	0	NULL	-0.76 V	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction potentials E ( 1/2 ) ( red ) cover a large range of -2.11 V for 2 , 5-diphenyl-1 , 3 , 4 - oxadiazole to -0.76 V for 1 , 2 , 3 , 4 , 5 , 6-hexa ( 5-phenyl-1 , 3 , 4 - oxadiazo-2-yl ) benzene .
	manualset3
162453	6	412045	7	NULL	NULL	0	NULL	1 , 2 , 3 , 4 , 5 , 6-hexa ( 5-phenyl-1 , 3 , 4 - oxadiazo-2-yl ) benzene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction potentials E ( 1/2 ) ( red ) cover a large range of -2.11 V for 2 , 5-diphenyl-1 , 3 , 4 - oxadiazole to -0.76 V for 1 , 2 , 3 , 4 , 5 , 6-hexa ( 5-phenyl-1 , 3 , 4 - oxadiazo-2-yl ) benzene .
	manualset3
163801	7	412045	7	NULL	NULL	0	NULL	large range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction potentials E ( 1/2 ) ( red ) cover a large range of -2.11 V for 2 , 5-diphenyl-1 , 3 , 4 - oxadiazole to -0.76 V for 1 , 2 , 3 , 4 , 5 , 6-hexa ( 5-phenyl-1 , 3 , 4 - oxadiazo-2-yl ) benzene .
	manualset3
162454	1	412046	7	NULL	NULL	0	NULL	Abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Abnormalities of left ventricular contraction in patients with mitral valve prolapse have suggested a myocardial factor in this disease .
	manualset3
162455	2	412046	7	NULL	NULL	0	NULL	left ventricular contraction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Abnormalities of left ventricular contraction in patients with mitral valve prolapse have suggested a myocardial factor in this disease .
	manualset3
162456	3	412046	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Abnormalities of left ventricular contraction in patients with mitral valve prolapse have suggested a myocardial factor in this disease .
	manualset3
162457	4	412046	7	NULL	NULL	NULL	NULL	mitral valve prolapse	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Abnormalities of left ventricular contraction in patients with mitral valve prolapse have suggested a myocardial factor in this disease .
	manualset3
162458	5	412046	7	NULL	NULL	0	NULL	myocardial factor	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Abnormalities of left ventricular contraction in patients with mitral valve prolapse have suggested a myocardial factor in this disease .
	manualset3
162459	6	412046	7	NULL	NULL	NULL	NULL	disease 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Abnormalities of left ventricular contraction in patients with mitral valve prolapse have suggested a myocardial factor in this disease .
	manualset3
162460	1	412047	7	NULL	NULL	0	NULL	region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The region contains four long open reading frames ( ORFs ) , the last of which represents a 1088-nucleotide fragment at the start of the ARV L gene .
	manualset3
162461	2	412047	7	NULL	NULL	0	NULL	 four long open reading frames ( ORFs )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The region contains four long open reading frames ( ORFs ) , the last of which represents a 1088-nucleotide fragment at the start of the ARV L gene .
	manualset3
162462	3	412047	7	NULL	NULL	0	NULL	1088-nucleotide fragment 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The region contains four long open reading frames ( ORFs ) , the last of which represents a 1088-nucleotide fragment at the start of the ARV L gene .
	manualset3
162463	4	412047	7	NULL	NULL	0	NULL	start	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The region contains four long open reading frames ( ORFs ) , the last of which represents a 1088-nucleotide fragment at the start of the ARV L gene .
	manualset3
162464	5	412047	7	NULL	NULL	0	NULL	ARV L gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The region contains four long open reading frames ( ORFs ) , the last of which represents a 1088-nucleotide fragment at the start of the ARV L gene .
	manualset3
162465	1	412048	7	NULL	NULL	0	NULL	region	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The region surrounding the VRN1 locus in perennial ryegrass showed microcolinearity to the corresponding region on chromosome 3 in Oryza sativa with conserved gene order and orientation , while the micro-colinearity to the corresponding region in Triticum monococcum was less conserved .
	manualset3
162466	2	412048	7	NULL	NULL	0	NULL	VRN1 locus	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The region surrounding the VRN1 locus in perennial ryegrass showed microcolinearity to the corresponding region on chromosome 3 in Oryza sativa with conserved gene order and orientation , while the micro-colinearity to the corresponding region in Triticum monococcum was less conserved .
	manualset3
162467	3	412048	7	NULL	NULL	0	NULL	perennial ryegrass	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The region surrounding the VRN1 locus in perennial ryegrass showed microcolinearity to the corresponding region on chromosome 3 in Oryza sativa with conserved gene order and orientation , while the micro-colinearity to the corresponding region in Triticum monococcum was less conserved .
	manualset3
162468	4	412048	7	NULL	NULL	NULL	NULL	microcolinearity	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The region surrounding the VRN1 locus in perennial ryegrass showed microcolinearity to the corresponding region on chromosome 3 in Oryza sativa with conserved gene order and orientation , while the micro-colinearity to the corresponding region in Triticum monococcum was less conserved .
	manualset3
162469	5	412048	7	NULL	NULL	0	NULL	 region	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The region surrounding the VRN1 locus in perennial ryegrass showed microcolinearity to the corresponding region on chromosome 3 in Oryza sativa with conserved gene order and orientation , while the micro-colinearity to the corresponding region in Triticum monococcum was less conserved .
	manualset3
162470	6	412048	7	NULL	NULL	0	NULL	chromosome 3	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The region surrounding the VRN1 locus in perennial ryegrass showed microcolinearity to the corresponding region on chromosome 3 in Oryza sativa with conserved gene order and orientation , while the micro-colinearity to the corresponding region in Triticum monococcum was less conserved .
	manualset3
162471	7	412048	7	NULL	NULL	0	NULL	Oryza sativa	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The region surrounding the VRN1 locus in perennial ryegrass showed microcolinearity to the corresponding region on chromosome 3 in Oryza sativa with conserved gene order and orientation , while the micro-colinearity to the corresponding region in Triticum monococcum was less conserved .
	manualset3
162472	8	412048	7	NULL	NULL	0	NULL	conserved gene order 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The region surrounding the VRN1 locus in perennial ryegrass showed microcolinearity to the corresponding region on chromosome 3 in Oryza sativa with conserved gene order and orientation , while the micro-colinearity to the corresponding region in Triticum monococcum was less conserved .
	manualset3
162473	9	412048	7	NULL	NULL	0	NULL	orientation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The region surrounding the VRN1 locus in perennial ryegrass showed microcolinearity to the corresponding region on chromosome 3 in Oryza sativa with conserved gene order and orientation , while the micro-colinearity to the corresponding region in Triticum monococcum was less conserved .
	manualset3
162474	10	412048	7	NULL	NULL	NULL	NULL	micro-colinearity 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The region surrounding the VRN1 locus in perennial ryegrass showed microcolinearity to the corresponding region on chromosome 3 in Oryza sativa with conserved gene order and orientation , while the micro-colinearity to the corresponding region in Triticum monococcum was less conserved .
	manualset3
162475	11	412048	7	NULL	NULL	0	NULL	region	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The region surrounding the VRN1 locus in perennial ryegrass showed microcolinearity to the corresponding region on chromosome 3 in Oryza sativa with conserved gene order and orientation , while the micro-colinearity to the corresponding region in Triticum monococcum was less conserved .
	manualset3
162476	12	412048	7	NULL	NULL	0	NULL	Triticum monococcum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The region surrounding the VRN1 locus in perennial ryegrass showed microcolinearity to the corresponding region on chromosome 3 in Oryza sativa with conserved gene order and orientation , while the micro-colinearity to the corresponding region in Triticum monococcum was less conserved .
	manualset3
162477	1	412049	7	NULL	NULL	0	NULL	regression equation	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The regression equation for estimated milk intake against measured milk intake across all ages was y = 0.988 x + 2.75 , r = 0.927 , n = 69 with 95 per cent prediction intervals of + / - 36 g for a range of intakes of 0-250 g. Rigorous control of data collection and taking account of the infant 's age suggest that the prediction intervals for individual estimates can be improved to + / - 18 g at 5 d , and + / - 27 g at 6 weeks and over .
	manualset3
162478	2	412049	7	NULL	NULL	NULL	NULL	estimated milk intake	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The regression equation for estimated milk intake against measured milk intake across all ages was y = 0.988 x + 2.75 , r = 0.927 , n = 69 with 95 per cent prediction intervals of + / - 36 g for a range of intakes of 0-250 g. Rigorous control of data collection and taking account of the infant 's age suggest that the prediction intervals for individual estimates can be improved to + / - 18 g at 5 d , and + / - 27 g at 6 weeks and over .
	manualset3
162479	3	412049	7	NULL	NULL	0	NULL	measured milk intake	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The regression equation for estimated milk intake against measured milk intake across all ages was y = 0.988 x + 2.75 , r = 0.927 , n = 69 with 95 per cent prediction intervals of + / - 36 g for a range of intakes of 0-250 g. Rigorous control of data collection and taking account of the infant 's age suggest that the prediction intervals for individual estimates can be improved to + / - 18 g at 5 d , and + / - 27 g at 6 weeks and over .
	manualset3
162480	4	412049	7	NULL	NULL	NULL	NULL	ages	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The regression equation for estimated milk intake against measured milk intake across all ages was y = 0.988 x + 2.75 , r = 0.927 , n = 69 with 95 per cent prediction intervals of + / - 36 g for a range of intakes of 0-250 g. Rigorous control of data collection and taking account of the infant 's age suggest that the prediction intervals for individual estimates can be improved to + / - 18 g at 5 d , and + / - 27 g at 6 weeks and over .
	manualset3
162481	5	412049	7	NULL	NULL	0	NULL	y = 0.988 x + 2.75	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The regression equation for estimated milk intake against measured milk intake across all ages was y = 0.988 x + 2.75 , r = 0.927 , n = 69 with 95 per cent prediction intervals of + / - 36 g for a range of intakes of 0-250 g. Rigorous control of data collection and taking account of the infant 's age suggest that the prediction intervals for individual estimates can be improved to + / - 18 g at 5 d , and + / - 27 g at 6 weeks and over .
	manualset3
162482	6	412049	7	NULL	NULL	0	NULL	 r = 0.927	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The regression equation for estimated milk intake against measured milk intake across all ages was y = 0.988 x + 2.75 , r = 0.927 , n = 69 with 95 per cent prediction intervals of + / - 36 g for a range of intakes of 0-250 g. Rigorous control of data collection and taking account of the infant 's age suggest that the prediction intervals for individual estimates can be improved to + / - 18 g at 5 d , and + / - 27 g at 6 weeks and over .
	manualset3
162483	7	412049	7	NULL	NULL	0	NULL	n = 69	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The regression equation for estimated milk intake against measured milk intake across all ages was y = 0.988 x + 2.75 , r = 0.927 , n = 69 with 95 per cent prediction intervals of + / - 36 g for a range of intakes of 0-250 g. Rigorous control of data collection and taking account of the infant 's age suggest that the prediction intervals for individual estimates can be improved to + / - 18 g at 5 d , and + / - 27 g at 6 weeks and over .
	manualset3
162484	8	412049	7	NULL	NULL	0	NULL	95 per cent 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The regression equation for estimated milk intake against measured milk intake across all ages was y = 0.988 x + 2.75 , r = 0.927 , n = 69 with 95 per cent prediction intervals of + / - 36 g for a range of intakes of 0-250 g. Rigorous control of data collection and taking account of the infant 's age suggest that the prediction intervals for individual estimates can be improved to + / - 18 g at 5 d , and + / - 27 g at 6 weeks and over .
	manualset3
162486	10	412049	7	NULL	NULL	NULL	NULL	prediction intervals of + / - 36 g 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The regression equation for estimated milk intake against measured milk intake across all ages was y = 0.988 x + 2.75 , r = 0.927 , n = 69 with 95 per cent prediction intervals of + / - 36 g for a range of intakes of 0-250 g. Rigorous control of data collection and taking account of the infant 's age suggest that the prediction intervals for individual estimates can be improved to + / - 18 g at 5 d , and + / - 27 g at 6 weeks and over .
	manualset3
162487	11	412049	7	NULL	NULL	0	NULL	 range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The regression equation for estimated milk intake against measured milk intake across all ages was y = 0.988 x + 2.75 , r = 0.927 , n = 69 with 95 per cent prediction intervals of + / - 36 g for a range of intakes of 0-250 g. Rigorous control of data collection and taking account of the infant 's age suggest that the prediction intervals for individual estimates can be improved to + / - 18 g at 5 d , and + / - 27 g at 6 weeks and over .
	manualset3
162488	12	412049	7	NULL	NULL	0	NULL	intakes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The regression equation for estimated milk intake against measured milk intake across all ages was y = 0.988 x + 2.75 , r = 0.927 , n = 69 with 95 per cent prediction intervals of + / - 36 g for a range of intakes of 0-250 g. Rigorous control of data collection and taking account of the infant 's age suggest that the prediction intervals for individual estimates can be improved to + / - 18 g at 5 d , and + / - 27 g at 6 weeks and over .
	manualset3
162489	13	412049	7	NULL	NULL	0	NULL	0-250 g	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The regression equation for estimated milk intake against measured milk intake across all ages was y = 0.988 x + 2.75 , r = 0.927 , n = 69 with 95 per cent prediction intervals of + / - 36 g for a range of intakes of 0-250 g. Rigorous control of data collection and taking account of the infant 's age suggest that the prediction intervals for individual estimates can be improved to + / - 18 g at 5 d , and + / - 27 g at 6 weeks and over .
	manualset3
162490	14	412049	7	NULL	NULL	0	NULL	Rigorous control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The regression equation for estimated milk intake against measured milk intake across all ages was y = 0.988 x + 2.75 , r = 0.927 , n = 69 with 95 per cent prediction intervals of + / - 36 g for a range of intakes of 0-250 g. Rigorous control of data collection and taking account of the infant 's age suggest that the prediction intervals for individual estimates can be improved to + / - 18 g at 5 d , and + / - 27 g at 6 weeks and over .
	manualset3
162491	15	412049	7	NULL	NULL	0	NULL	data collection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The regression equation for estimated milk intake against measured milk intake across all ages was y = 0.988 x + 2.75 , r = 0.927 , n = 69 with 95 per cent prediction intervals of + / - 36 g for a range of intakes of 0-250 g. Rigorous control of data collection and taking account of the infant 's age suggest that the prediction intervals for individual estimates can be improved to + / - 18 g at 5 d , and + / - 27 g at 6 weeks and over .
	manualset3
162492	16	412049	7	NULL	NULL	0	NULL	 infant 's age	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The regression equation for estimated milk intake against measured milk intake across all ages was y = 0.988 x + 2.75 , r = 0.927 , n = 69 with 95 per cent prediction intervals of + / - 36 g for a range of intakes of 0-250 g. Rigorous control of data collection and taking account of the infant 's age suggest that the prediction intervals for individual estimates can be improved to + / - 18 g at 5 d , and + / - 27 g at 6 weeks and over .
	manualset3
162493	17	412049	7	NULL	NULL	NULL	NULL	prediction intervals	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The regression equation for estimated milk intake against measured milk intake across all ages was y = 0.988 x + 2.75 , r = 0.927 , n = 69 with 95 per cent prediction intervals of + / - 36 g for a range of intakes of 0-250 g. Rigorous control of data collection and taking account of the infant 's age suggest that the prediction intervals for individual estimates can be improved to + / - 18 g at 5 d , and + / - 27 g at 6 weeks and over .
	manualset3
162494	18	412049	7	NULL	NULL	0	NULL	+ / - 18 g 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The regression equation for estimated milk intake against measured milk intake across all ages was y = 0.988 x + 2.75 , r = 0.927 , n = 69 with 95 per cent prediction intervals of + / - 36 g for a range of intakes of 0-250 g. Rigorous control of data collection and taking account of the infant 's age suggest that the prediction intervals for individual estimates can be improved to + / - 18 g at 5 d , and + / - 27 g at 6 weeks and over .
	manualset3
162495	19	412049	7	NULL	NULL	0	NULL	5 d 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The regression equation for estimated milk intake against measured milk intake across all ages was y = 0.988 x + 2.75 , r = 0.927 , n = 69 with 95 per cent prediction intervals of + / - 36 g for a range of intakes of 0-250 g. Rigorous control of data collection and taking account of the infant 's age suggest that the prediction intervals for individual estimates can be improved to + / - 18 g at 5 d , and + / - 27 g at 6 weeks and over .
	manualset3
162496	20	412049	7	NULL	NULL	0	NULL	+ / - 27 g 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The regression equation for estimated milk intake against measured milk intake across all ages was y = 0.988 x + 2.75 , r = 0.927 , n = 69 with 95 per cent prediction intervals of + / - 36 g for a range of intakes of 0-250 g. Rigorous control of data collection and taking account of the infant 's age suggest that the prediction intervals for individual estimates can be improved to + / - 18 g at 5 d , and + / - 27 g at 6 weeks and over .
	manualset3
162497	21	412049	7	NULL	NULL	0	NULL	 6 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The regression equation for estimated milk intake against measured milk intake across all ages was y = 0.988 x + 2.75 , r = 0.927 , n = 69 with 95 per cent prediction intervals of + / - 36 g for a range of intakes of 0-250 g. Rigorous control of data collection and taking account of the infant 's age suggest that the prediction intervals for individual estimates can be improved to + / - 18 g at 5 d , and + / - 27 g at 6 weeks and over .
	manualset3
163802	22	412049	7	NULL	NULL	0	NULL	individual estimates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The regression equation for estimated milk intake against measured milk intake across all ages was y = 0.988 x + 2.75 , r = 0.927 , n = 69 with 95 per cent prediction intervals of + / - 36 g for a range of intakes of 0-250 g. Rigorous control of data collection and taking account of the infant 's age suggest that the prediction intervals for individual estimates can be improved to + / - 18 g at 5 d , and + / - 27 g at 6 weeks and over .
	manualset3
162498	1	412050	7	NULL	NULL	NULL	NULL	regulation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The regulation of E2F transcription factors is closely associated with the function of the retinoblastoma family of tumor suppressors ( RB pathway ) .
	manualset3
162499	2	412050	7	NULL	NULL	0	NULL	E2F transcription factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of E2F transcription factors is closely associated with the function of the retinoblastoma family of tumor suppressors ( RB pathway ) .
	manualset3
162500	3	412050	7	NULL	NULL	0	NULL	function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of E2F transcription factors is closely associated with the function of the retinoblastoma family of tumor suppressors ( RB pathway ) .
	manualset3
162501	4	412050	7	NULL	NULL	0	NULL	retinoblastoma family of tumor suppressors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of E2F transcription factors is closely associated with the function of the retinoblastoma family of tumor suppressors ( RB pathway ) .
	manualset3
162502	5	412050	7	NULL	NULL	0	NULL	RB pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of E2F transcription factors is closely associated with the function of the retinoblastoma family of tumor suppressors ( RB pathway ) .
	manualset3
162503	1	412051	7	NULL	NULL	0	NULL	 regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of avian lipoprotein lipase by dibutyryl cyclic AMP in cultured adipocytes was studied with quantitative and specific methods for the measurements of enzyme catalytic activity , enzyme protein mass , and immunoadsorption of labeled enzyme .
	manualset3
162504	2	412051	7	NULL	NULL	0	NULL	avian lipoprotein lipase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of avian lipoprotein lipase by dibutyryl cyclic AMP in cultured adipocytes was studied with quantitative and specific methods for the measurements of enzyme catalytic activity , enzyme protein mass , and immunoadsorption of labeled enzyme .
	manualset3
162505	3	412051	7	NULL	NULL	0	NULL	dibutyryl cyclic AMP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of avian lipoprotein lipase by dibutyryl cyclic AMP in cultured adipocytes was studied with quantitative and specific methods for the measurements of enzyme catalytic activity , enzyme protein mass , and immunoadsorption of labeled enzyme .
	manualset3
162506	4	412051	7	NULL	NULL	0	NULL	cultured adipocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of avian lipoprotein lipase by dibutyryl cyclic AMP in cultured adipocytes was studied with quantitative and specific methods for the measurements of enzyme catalytic activity , enzyme protein mass , and immunoadsorption of labeled enzyme .
	manualset3
162510	5	412051	7	NULL	NULL	0	NULL	specific methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of avian lipoprotein lipase by dibutyryl cyclic AMP in cultured adipocytes was studied with quantitative and specific methods for the measurements of enzyme catalytic activity , enzyme protein mass , and immunoadsorption of labeled enzyme .
	manualset3
162511	6	412051	7	NULL	NULL	0	NULL	 measurements	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of avian lipoprotein lipase by dibutyryl cyclic AMP in cultured adipocytes was studied with quantitative and specific methods for the measurements of enzyme catalytic activity , enzyme protein mass , and immunoadsorption of labeled enzyme .
	manualset3
162512	7	412051	7	NULL	NULL	0	NULL	enzyme catalytic activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of avian lipoprotein lipase by dibutyryl cyclic AMP in cultured adipocytes was studied with quantitative and specific methods for the measurements of enzyme catalytic activity , enzyme protein mass , and immunoadsorption of labeled enzyme .
	manualset3
162513	8	412051	7	NULL	NULL	0	NULL	enzyme protein mass	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of avian lipoprotein lipase by dibutyryl cyclic AMP in cultured adipocytes was studied with quantitative and specific methods for the measurements of enzyme catalytic activity , enzyme protein mass , and immunoadsorption of labeled enzyme .
	manualset3
162514	9	412051	7	NULL	NULL	0	NULL	immunoadsorption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of avian lipoprotein lipase by dibutyryl cyclic AMP in cultured adipocytes was studied with quantitative and specific methods for the measurements of enzyme catalytic activity , enzyme protein mass , and immunoadsorption of labeled enzyme .
	manualset3
162515	10	412051	7	NULL	NULL	0	NULL	labeled enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of avian lipoprotein lipase by dibutyryl cyclic AMP in cultured adipocytes was studied with quantitative and specific methods for the measurements of enzyme catalytic activity , enzyme protein mass , and immunoadsorption of labeled enzyme .
	manualset3
162516	1	412052	7	NULL	NULL	0	NULL	regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of cytoplasmic calcium is a key process in nerve tissue .
	manualset3
162518	2	412052	7	NULL	NULL	0	NULL	cytoplasmic calcium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of cytoplasmic calcium is a key process in nerve tissue .
	manualset3
162519	3	412052	7	NULL	NULL	0	NULL	process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of cytoplasmic calcium is a key process in nerve tissue .
	manualset3
162520	4	412052	7	NULL	NULL	0	NULL	 nerve tissue	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of cytoplasmic calcium is a key process in nerve tissue .
	manualset3
162521	1	412053	7	NULL	NULL	NULL	NULL	regulatory effect	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The regulatory effect of galectin-1 is mediated , in part , through its ability to induce , in an Id3 ( inhibitor of DNA binding 3 ) - dependent manner , the expression of IL-10 in monocytes and MdDCs .
	manualset3
162522	2	412053	7	NULL	NULL	0	NULL	galectin-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulatory effect of galectin-1 is mediated , in part , through its ability to induce , in an Id3 ( inhibitor of DNA binding 3 ) - dependent manner , the expression of IL-10 in monocytes and MdDCs .
	manualset3
162523	3	412053	7	NULL	NULL	0	NULL	Id3 ( inhibitor of DNA binding 3 ) - dependent manner	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulatory effect of galectin-1 is mediated , in part , through its ability to induce , in an Id3 ( inhibitor of DNA binding 3 ) - dependent manner , the expression of IL-10 in monocytes and MdDCs .
	manualset3
162524	4	412053	7	NULL	NULL	0	NULL	expression of IL-10	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulatory effect of galectin-1 is mediated , in part , through its ability to induce , in an Id3 ( inhibitor of DNA binding 3 ) - dependent manner , the expression of IL-10 in monocytes and MdDCs .
	manualset3
162525	5	412053	7	NULL	NULL	0	NULL	 monocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulatory effect of galectin-1 is mediated , in part , through its ability to induce , in an Id3 ( inhibitor of DNA binding 3 ) - dependent manner , the expression of IL-10 in monocytes and MdDCs .
	manualset3
162526	6	412053	7	NULL	NULL	0	NULL	MdDCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulatory effect of galectin-1 is mediated , in part , through its ability to induce , in an Id3 ( inhibitor of DNA binding 3 ) - dependent manner , the expression of IL-10 in monocytes and MdDCs .
	manualset3
162527	1	412054	7	NULL	NULL	NULL	NULL	reinforced zirconia ceramics	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reinforced zirconia ceramics allow fabrication of durable esthetic restorations in cases with high functional loading and the unification of the post , core , and crown in a single unit decreases the frequency of failure by creating a monobloc effect .
	manualset3
162528	2	412054	7	NULL	NULL	0	NULL	fabrication	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The reinforced zirconia ceramics allow fabrication of durable esthetic restorations in cases with high functional loading and the unification of the post , core , and crown in a single unit decreases the frequency of failure by creating a monobloc effect .
	manualset3
162529	3	412054	7	NULL	NULL	NULL	NULL	durable esthetic restorations	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reinforced zirconia ceramics allow fabrication of durable esthetic restorations in cases with high functional loading and the unification of the post , core , and crown in a single unit decreases the frequency of failure by creating a monobloc effect .
	manualset3
162530	4	412054	7	NULL	NULL	0	NULL	high functional loading	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The reinforced zirconia ceramics allow fabrication of durable esthetic restorations in cases with high functional loading and the unification of the post , core , and crown in a single unit decreases the frequency of failure by creating a monobloc effect .
	manualset3
162531	5	412054	7	NULL	NULL	NULL	NULL	unification 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reinforced zirconia ceramics allow fabrication of durable esthetic restorations in cases with high functional loading and the unification of the post , core , and crown in a single unit decreases the frequency of failure by creating a monobloc effect .
	manualset3
162532	6	412054	7	NULL	NULL	NULL	NULL	 core	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reinforced zirconia ceramics allow fabrication of durable esthetic restorations in cases with high functional loading and the unification of the post , core , and crown in a single unit decreases the frequency of failure by creating a monobloc effect .
	manualset3
162533	7	412054	7	NULL	NULL	NULL	NULL	crown	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reinforced zirconia ceramics allow fabrication of durable esthetic restorations in cases with high functional loading and the unification of the post , core , and crown in a single unit decreases the frequency of failure by creating a monobloc effect .
	manualset3
162534	8	412054	7	NULL	NULL	NULL	NULL	 frequency	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reinforced zirconia ceramics allow fabrication of durable esthetic restorations in cases with high functional loading and the unification of the post , core , and crown in a single unit decreases the frequency of failure by creating a monobloc effect .
	manualset3
162535	10	412054	7	NULL	NULL	NULL	NULL	monobloc effect	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reinforced zirconia ceramics allow fabrication of durable esthetic restorations in cases with high functional loading and the unification of the post , core , and crown in a single unit decreases the frequency of failure by creating a monobloc effect .
	manualset3
163803	9	412054	7	NULL	NULL	0	NULL	failure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The reinforced zirconia ceramics allow fabrication of durable esthetic restorations in cases with high functional loading and the unification of the post , core , and crown in a single unit decreases the frequency of failure by creating a monobloc effect .
	manualset3
163804	11	412054	7	NULL	NULL	NULL	NULL	cases	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reinforced zirconia ceramics allow fabrication of durable esthetic restorations in cases with high functional loading and the unification of the post , core , and crown in a single unit decreases the frequency of failure by creating a monobloc effect .
	manualset3
164152	12	412054	7	NULL	NULL	0	NULL	 post	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The reinforced zirconia ceramics allow fabrication of durable esthetic restorations in cases with high functional loading and the unification of the post , core , and crown in a single unit decreases the frequency of failure by creating a monobloc effect .
	manualset3
164153	13	412054	7	NULL	NULL	0	NULL	single unit	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The reinforced zirconia ceramics allow fabrication of durable esthetic restorations in cases with high functional loading and the unification of the post , core , and crown in a single unit decreases the frequency of failure by creating a monobloc effect .
	manualset3
162536	1	412055	7	NULL	NULL	0	NULL	rejection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The rejection of neovascularized pig proislet ( islet precursor ) xenografts in mice is a CD4 T cell-dependent process involving invasion of the graft site mainly by host CD4 T cells and eosinophils .
	manualset3
162537	2	412055	7	NULL	NULL	0	NULL	neovascularized pig proislet ( islet precursor ) xenografts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The rejection of neovascularized pig proislet ( islet precursor ) xenografts in mice is a CD4 T cell-dependent process involving invasion of the graft site mainly by host CD4 T cells and eosinophils .
	manualset3
162538	3	412055	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The rejection of neovascularized pig proislet ( islet precursor ) xenografts in mice is a CD4 T cell-dependent process involving invasion of the graft site mainly by host CD4 T cells and eosinophils .
	manualset3
162539	4	412055	7	NULL	NULL	NULL	NULL	CD4 T cell-dependent process 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The rejection of neovascularized pig proislet ( islet precursor ) xenografts in mice is a CD4 T cell-dependent process involving invasion of the graft site mainly by host CD4 T cells and eosinophils .
	manualset3
162540	5	412055	7	NULL	NULL	0	NULL	invasion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The rejection of neovascularized pig proislet ( islet precursor ) xenografts in mice is a CD4 T cell-dependent process involving invasion of the graft site mainly by host CD4 T cells and eosinophils .
	manualset3
162541	6	412055	7	NULL	NULL	0	NULL	 graft site	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The rejection of neovascularized pig proislet ( islet precursor ) xenografts in mice is a CD4 T cell-dependent process involving invasion of the graft site mainly by host CD4 T cells and eosinophils .
	manualset3
162542	7	412055	7	NULL	NULL	0	NULL	host CD4 T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The rejection of neovascularized pig proislet ( islet precursor ) xenografts in mice is a CD4 T cell-dependent process involving invasion of the graft site mainly by host CD4 T cells and eosinophils .
	manualset3
162543	8	412055	7	NULL	NULL	0	NULL	eosinophils	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The rejection of neovascularized pig proislet ( islet precursor ) xenografts in mice is a CD4 T cell-dependent process involving invasion of the graft site mainly by host CD4 T cells and eosinophils .
	manualset3
162544	1	412056	7	NULL	NULL	0	NULL	relapse rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The relapse rate was 8 % ( 9/108 ) for the CQ group and 3 % ( 4/132 ) for the comparison group ( P = 0.07 ) .
	manualset3
162545	2	412056	7	NULL	NULL	NULL	NULL	8 % ( 9/108 )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relapse rate was 8 % ( 9/108 ) for the CQ group and 3 % ( 4/132 ) for the comparison group ( P = 0.07 ) .
	manualset3
162546	3	412056	7	NULL	NULL	0	NULL	CQ group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The relapse rate was 8 % ( 9/108 ) for the CQ group and 3 % ( 4/132 ) for the comparison group ( P = 0.07 ) .
	manualset3
162547	4	412056	7	NULL	NULL	0	NULL	3 % ( 4/132 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The relapse rate was 8 % ( 9/108 ) for the CQ group and 3 % ( 4/132 ) for the comparison group ( P = 0.07 ) .
	manualset3
162548	5	412056	7	NULL	NULL	0	NULL	comparison group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The relapse rate was 8 % ( 9/108 ) for the CQ group and 3 % ( 4/132 ) for the comparison group ( P = 0.07 ) .
	manualset3
162549	6	412056	7	NULL	NULL	0	NULL	P = 0.07	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The relapse rate was 8 % ( 9/108 ) for the CQ group and 3 % ( 4/132 ) for the comparison group ( P = 0.07 ) .
	manualset3
162550	1	412057	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The relation between cannabis use and dependence on one hand and anxious and depressive symptomatology on the other hand may have been obscured by the acute mood effect of cannabis consumption .
	manualset3
162551	2	412057	7	NULL	NULL	NULL	NULL	cannabis use	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relation between cannabis use and dependence on one hand and anxious and depressive symptomatology on the other hand may have been obscured by the acute mood effect of cannabis consumption .
	manualset3
162552	3	412057	7	NULL	NULL	0	NULL	anxious symptomatology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The relation between cannabis use and dependence on one hand and anxious and depressive symptomatology on the other hand may have been obscured by the acute mood effect of cannabis consumption .
	manualset3
162553	4	412057	7	NULL	NULL	0	NULL	depressive symptomatology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The relation between cannabis use and dependence on one hand and anxious and depressive symptomatology on the other hand may have been obscured by the acute mood effect of cannabis consumption .
	manualset3
162554	5	412057	7	NULL	NULL	0	NULL	acute mood effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The relation between cannabis use and dependence on one hand and anxious and depressive symptomatology on the other hand may have been obscured by the acute mood effect of cannabis consumption .
	manualset3
162555	6	412057	7	NULL	NULL	NULL	NULL	cannabis consumption	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relation between cannabis use and dependence on one hand and anxious and depressive symptomatology on the other hand may have been obscured by the acute mood effect of cannabis consumption .
	manualset3
169724	7	412057	7	NULL	NULL	0	NULL	cannabis dependence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The relation between cannabis use and dependence on one hand and anxious and depressive symptomatology on the other hand may have been obscured by the acute mood effect of cannabis consumption .
	manualset3
162556	1	412058	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The relation between the rod and cone mechanisms in the after-effect of seen movement .
	manualset3
162557	2	412058	7	NULL	NULL	0	NULL	rod mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relation between the rod and cone mechanisms in the after-effect of seen movement .
	manualset3
162558	3	412058	7	NULL	NULL	0	NULL	cone mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relation between the rod and cone mechanisms in the after-effect of seen movement .
	manualset3
162559	4	412058	7	NULL	NULL	0	NULL	after-effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relation between the rod and cone mechanisms in the after-effect of seen movement .
	manualset3
162560	5	412058	7	NULL	NULL	0	NULL	movement	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relation between the rod and cone mechanisms in the after-effect of seen movement .
	manualset3
162561	1	412059	7	NULL	NULL	0	NULL	 relation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The relation of extraarticular tenderness to inflammatory joint disease and personality in patients with rheumatoid arthritis .
	manualset3
162563	3	412059	7	NULL	NULL	0	NULL	inflammatory joint disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The relation of extraarticular tenderness to inflammatory joint disease and personality in patients with rheumatoid arthritis .
	manualset3
162564	4	412059	7	NULL	NULL	NULL	NULL	personality	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relation of extraarticular tenderness to inflammatory joint disease and personality in patients with rheumatoid arthritis .
	manualset3
162565	5	412059	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The relation of extraarticular tenderness to inflammatory joint disease and personality in patients with rheumatoid arthritis .
	manualset3
162566	6	412059	7	NULL	NULL	0	NULL	rheumatoid arthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The relation of extraarticular tenderness to inflammatory joint disease and personality in patients with rheumatoid arthritis .
	manualset3
163805	2	412059	7	NULL	NULL	0	NULL	extraarticular tenderness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The relation of extraarticular tenderness to inflammatory joint disease and personality in patients with rheumatoid arthritis .
	manualset3
162567	1	412060	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between Alzheimer disease ( AD ) and dementia with Lewy bodies ( senile dementia Lewy body type , or SDLT ) and dementia in Parkinson 's disease is unclear .
	manualset3
162568	2	412060	7	NULL	NULL	0	NULL	Alzheimer disease ( AD ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between Alzheimer disease ( AD ) and dementia with Lewy bodies ( senile dementia Lewy body type , or SDLT ) and dementia in Parkinson 's disease is unclear .
	manualset3
162569	3	412060	7	NULL	NULL	0	NULL	dementia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between Alzheimer disease ( AD ) and dementia with Lewy bodies ( senile dementia Lewy body type , or SDLT ) and dementia in Parkinson 's disease is unclear .
	manualset3
162570	4	412060	7	NULL	NULL	NULL	NULL	Lewy bodies	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relationship between Alzheimer disease ( AD ) and dementia with Lewy bodies ( senile dementia Lewy body type , or SDLT ) and dementia in Parkinson 's disease is unclear .
	manualset3
162571	5	412060	7	NULL	NULL	0	NULL	senile dementia Lewy body type , or SDLT	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between Alzheimer disease ( AD ) and dementia with Lewy bodies ( senile dementia Lewy body type , or SDLT ) and dementia in Parkinson 's disease is unclear .
	manualset3
162572	6	412060	7	NULL	NULL	0	NULL	dementia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between Alzheimer disease ( AD ) and dementia with Lewy bodies ( senile dementia Lewy body type , or SDLT ) and dementia in Parkinson 's disease is unclear .
	manualset3
162573	7	412060	7	NULL	NULL	0	NULL	Parkinson 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between Alzheimer disease ( AD ) and dementia with Lewy bodies ( senile dementia Lewy body type , or SDLT ) and dementia in Parkinson 's disease is unclear .
	manualset3
162574	1	412061	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between connexins , gap junctions , tissue architecture and tumor invasion , as studied in a novel in vitro model of HPV-16-associated cervical cancer progression .
	manualset3
162575	2	412061	7	NULL	NULL	0	NULL	connexins 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between connexins , gap junctions , tissue architecture and tumor invasion , as studied in a novel in vitro model of HPV-16-associated cervical cancer progression .
	manualset3
162576	3	412061	7	NULL	NULL	0	NULL	gap junctions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between connexins , gap junctions , tissue architecture and tumor invasion , as studied in a novel in vitro model of HPV-16-associated cervical cancer progression .
	manualset3
162577	4	412061	7	NULL	NULL	0	NULL	tissue architecture	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between connexins , gap junctions , tissue architecture and tumor invasion , as studied in a novel in vitro model of HPV-16-associated cervical cancer progression .
	manualset3
162578	5	412061	7	NULL	NULL	0	NULL	tumor invasion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between connexins , gap junctions , tissue architecture and tumor invasion , as studied in a novel in vitro model of HPV-16-associated cervical cancer progression .
	manualset3
162579	6	412061	7	NULL	NULL	0	NULL	novel in vitro model	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between connexins , gap junctions , tissue architecture and tumor invasion , as studied in a novel in vitro model of HPV-16-associated cervical cancer progression .
	manualset3
162580	7	412061	7	NULL	NULL	NULL	NULL	HPV-16-associated cervical cancer progression	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relationship between connexins , gap junctions , tissue architecture and tumor invasion , as studied in a novel in vitro model of HPV-16-associated cervical cancer progression .
	manualset3
162582	1	412062	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between insulin autoantibodies and islet cell histology in the diabetes prone BB rat .
	manualset3
162583	2	412062	7	NULL	NULL	0	NULL	insulin autoantibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between insulin autoantibodies and islet cell histology in the diabetes prone BB rat .
	manualset3
162584	3	412062	7	NULL	NULL	0	NULL	islet cell histology	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between insulin autoantibodies and islet cell histology in the diabetes prone BB rat .
	manualset3
162585	4	412062	7	NULL	NULL	0	NULL	 diabetes prone BB rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between insulin autoantibodies and islet cell histology in the diabetes prone BB rat .
	manualset3
162586	1	412063	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between interception fraction and corn biomass was accurately approximated by a filtration model with an absorption coefficient of 3.60 m2 kg-1 .
	manualset3
162587	2	412063	7	NULL	NULL	0	NULL	interception fraction	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between interception fraction and corn biomass was accurately approximated by a filtration model with an absorption coefficient of 3.60 m2 kg-1 .
	manualset3
162588	3	412063	7	NULL	NULL	0	NULL	corn biomass	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between interception fraction and corn biomass was accurately approximated by a filtration model with an absorption coefficient of 3.60 m2 kg-1 .
	manualset3
162589	4	412063	7	NULL	NULL	0	NULL	filtration model	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between interception fraction and corn biomass was accurately approximated by a filtration model with an absorption coefficient of 3.60 m2 kg-1 .
	manualset3
162590	5	412063	7	NULL	NULL	0	NULL	absorption coefficient	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between interception fraction and corn biomass was accurately approximated by a filtration model with an absorption coefficient of 3.60 m2 kg-1 .
	manualset3
162591	6	412063	7	NULL	NULL	0	NULL	3.60 m2 kg-1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between interception fraction and corn biomass was accurately approximated by a filtration model with an absorption coefficient of 3.60 m2 kg-1 .
	manualset3
162592	1	412064	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between oxygen uptake reserve and heart rate reserve is affected by intensity and duration during aerobic exercise at constant work rate .
	manualset3
162593	2	412064	7	NULL	NULL	NULL	NULL	oxygen uptake reserve	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relationship between oxygen uptake reserve and heart rate reserve is affected by intensity and duration during aerobic exercise at constant work rate .
	manualset3
162594	3	412064	7	NULL	NULL	0	NULL	heart rate reserve	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between oxygen uptake reserve and heart rate reserve is affected by intensity and duration during aerobic exercise at constant work rate .
	manualset3
162595	4	412064	7	NULL	NULL	0	NULL	 intensity 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between oxygen uptake reserve and heart rate reserve is affected by intensity and duration during aerobic exercise at constant work rate .
	manualset3
162596	5	412064	7	NULL	NULL	0	NULL	duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between oxygen uptake reserve and heart rate reserve is affected by intensity and duration during aerobic exercise at constant work rate .
	manualset3
162597	6	412064	7	NULL	NULL	0	NULL	aerobic exercise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between oxygen uptake reserve and heart rate reserve is affected by intensity and duration during aerobic exercise at constant work rate .
	manualset3
162598	7	412064	7	NULL	NULL	0	NULL	constant work rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between oxygen uptake reserve and heart rate reserve is affected by intensity and duration during aerobic exercise at constant work rate .
	manualset3
162599	1	412065	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between p53 gene expression and DNA content in advanced gallbladder carcinoma was studied .
	manualset3
162600	2	412065	7	NULL	NULL	0	NULL	p53 gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between p53 gene expression and DNA content in advanced gallbladder carcinoma was studied .
	manualset3
162601	3	412065	7	NULL	NULL	0	NULL	DNA content	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between p53 gene expression and DNA content in advanced gallbladder carcinoma was studied .
	manualset3
162602	4	412065	7	NULL	NULL	0	NULL	advanced gallbladder carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between p53 gene expression and DNA content in advanced gallbladder carcinoma was studied .
	manualset3
162603	1	412066	7	NULL	NULL	0	NULL	 relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between prior alcohol consumption and the risk of breast cancer was studied in 1954 women in the Tecumseh Community Health Study ( TCHS ) who entered the cohort in 1959-1960 and were followed potentially for 28 years .
	manualset3
162604	2	412066	7	NULL	NULL	NULL	NULL	alcohol consumption	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relationship between prior alcohol consumption and the risk of breast cancer was studied in 1954 women in the Tecumseh Community Health Study ( TCHS ) who entered the cohort in 1959-1960 and were followed potentially for 28 years .
	manualset3
162605	3	412066	7	NULL	NULL	0	NULL	 risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between prior alcohol consumption and the risk of breast cancer was studied in 1954 women in the Tecumseh Community Health Study ( TCHS ) who entered the cohort in 1959-1960 and were followed potentially for 28 years .
	manualset3
162606	4	412066	7	NULL	NULL	0	NULL	breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between prior alcohol consumption and the risk of breast cancer was studied in 1954 women in the Tecumseh Community Health Study ( TCHS ) who entered the cohort in 1959-1960 and were followed potentially for 28 years .
	manualset3
162608	6	412066	7	NULL	NULL	NULL	NULL	1954 women	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relationship between prior alcohol consumption and the risk of breast cancer was studied in 1954 women in the Tecumseh Community Health Study ( TCHS ) who entered the cohort in 1959-1960 and were followed potentially for 28 years .
	manualset3
162609	7	412066	7	NULL	NULL	NULL	NULL	Tecumseh Community Health Study ( TCHS )	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relationship between prior alcohol consumption and the risk of breast cancer was studied in 1954 women in the Tecumseh Community Health Study ( TCHS ) who entered the cohort in 1959-1960 and were followed potentially for 28 years .
	manualset3
162610	8	412066	7	NULL	NULL	0	NULL	cohort	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between prior alcohol consumption and the risk of breast cancer was studied in 1954 women in the Tecumseh Community Health Study ( TCHS ) who entered the cohort in 1959-1960 and were followed potentially for 28 years .
	manualset3
162611	9	412066	7	NULL	NULL	NULL	NULL	1959-1960	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relationship between prior alcohol consumption and the risk of breast cancer was studied in 1954 women in the Tecumseh Community Health Study ( TCHS ) who entered the cohort in 1959-1960 and were followed potentially for 28 years .
	manualset3
162612	10	412066	7	NULL	NULL	0	NULL	28 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between prior alcohol consumption and the risk of breast cancer was studied in 1954 women in the Tecumseh Community Health Study ( TCHS ) who entered the cohort in 1959-1960 and were followed potentially for 28 years .
	manualset3
162613	1	412067	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between psychosocial status and adequacy of GWG is significantly impacted by maternal sociodemographic factors and health practices engaged in during pregnancy .
	manualset3
162614	2	412067	7	NULL	NULL	NULL	NULL	psychosocial status	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relationship between psychosocial status and adequacy of GWG is significantly impacted by maternal sociodemographic factors and health practices engaged in during pregnancy .
	manualset3
162615	3	412067	7	NULL	NULL	NULL	NULL	GWG	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relationship between psychosocial status and adequacy of GWG is significantly impacted by maternal sociodemographic factors and health practices engaged in during pregnancy .
	manualset3
162616	4	412067	7	NULL	NULL	NULL	NULL	maternal sociodemographic factors	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relationship between psychosocial status and adequacy of GWG is significantly impacted by maternal sociodemographic factors and health practices engaged in during pregnancy .
	manualset3
162617	5	412067	7	NULL	NULL	NULL	NULL	health practices	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relationship between psychosocial status and adequacy of GWG is significantly impacted by maternal sociodemographic factors and health practices engaged in during pregnancy .
	manualset3
162618	6	412067	7	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between psychosocial status and adequacy of GWG is significantly impacted by maternal sociodemographic factors and health practices engaged in during pregnancy .
	manualset3
164154	7	412067	7	NULL	NULL	0	NULL	adequacy	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between psychosocial status and adequacy of GWG is significantly impacted by maternal sociodemographic factors and health practices engaged in during pregnancy .
	manualset3
162619	1	412068	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between running velocity and trunk rotation during normal running and running while dribbling was investigated in 7 male competitive basketball players and 7 male nonplayers .
	manualset3
162620	2	412068	7	NULL	NULL	0	NULL	running velocity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between running velocity and trunk rotation during normal running and running while dribbling was investigated in 7 male competitive basketball players and 7 male nonplayers .
	manualset3
162621	3	412068	7	NULL	NULL	0	NULL	trunk rotation	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between running velocity and trunk rotation during normal running and running while dribbling was investigated in 7 male competitive basketball players and 7 male nonplayers .
	manualset3
162622	4	412068	7	NULL	NULL	0	NULL	normal running	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between running velocity and trunk rotation during normal running and running while dribbling was investigated in 7 male competitive basketball players and 7 male nonplayers .
	manualset3
162623	5	412068	7	NULL	NULL	0	NULL	running while dribbling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between running velocity and trunk rotation during normal running and running while dribbling was investigated in 7 male competitive basketball players and 7 male nonplayers .
	manualset3
162624	6	412068	7	NULL	NULL	0	NULL	7 male competitive basketball players	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between running velocity and trunk rotation during normal running and running while dribbling was investigated in 7 male competitive basketball players and 7 male nonplayers .
	manualset3
162625	7	412068	7	NULL	NULL	0	NULL	7 male nonplayers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between running velocity and trunk rotation during normal running and running while dribbling was investigated in 7 male competitive basketball players and 7 male nonplayers .
	manualset3
162626	1	412069	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between structure and ability to circumvent cis-diamminedichloroplatinum ( II ) and/or trans-1R , 2 R-1S , 2 S - diaminocyclohexanetetrachloroplatinum ( IV ) resistance was complex .
	manualset3
162627	2	412069	7	NULL	NULL	0	NULL	structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between structure and ability to circumvent cis-diamminedichloroplatinum ( II ) and/or trans-1R , 2 R-1S , 2 S - diaminocyclohexanetetrachloroplatinum ( IV ) resistance was complex .
	manualset3
162628	3	412069	7	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between structure and ability to circumvent cis-diamminedichloroplatinum ( II ) and/or trans-1R , 2 R-1S , 2 S - diaminocyclohexanetetrachloroplatinum ( IV ) resistance was complex .
	manualset3
162629	4	412069	7	NULL	NULL	0	NULL	cis-diamminedichloroplatinum ( II )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between structure and ability to circumvent cis-diamminedichloroplatinum ( II ) and/or trans-1R , 2 R-1S , 2 S - diaminocyclohexanetetrachloroplatinum ( IV ) resistance was complex .
	manualset3
162630	5	412069	7	NULL	NULL	0	NULL	trans-1R , 2 R-1S , 2 S - diaminocyclohexanetetrachloroplatinum ( IV )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between structure and ability to circumvent cis-diamminedichloroplatinum ( II ) and/or trans-1R , 2 R-1S , 2 S - diaminocyclohexanetetrachloroplatinum ( IV ) resistance was complex .
	manualset3
162631	6	412069	7	NULL	NULL	0	NULL	resistance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between structure and ability to circumvent cis-diamminedichloroplatinum ( II ) and/or trans-1R , 2 R-1S , 2 S - diaminocyclohexanetetrachloroplatinum ( IV ) resistance was complex .
	manualset3
162632	1	412070	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between the volume of an intraocular gas bubble and the area of retina covered by the bubble was studied with the use of both a transparent model and a mathematical model of the vitreous cavity .
	manualset3
162633	2	412070	7	NULL	NULL	0	NULL	volume	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between the volume of an intraocular gas bubble and the area of retina covered by the bubble was studied with the use of both a transparent model and a mathematical model of the vitreous cavity .
	manualset3
162634	3	412070	7	NULL	NULL	NULL	NULL	intraocular gas bubble	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relationship between the volume of an intraocular gas bubble and the area of retina covered by the bubble was studied with the use of both a transparent model and a mathematical model of the vitreous cavity .
	manualset3
162635	4	412070	7	NULL	NULL	0	NULL	area of retina	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between the volume of an intraocular gas bubble and the area of retina covered by the bubble was studied with the use of both a transparent model and a mathematical model of the vitreous cavity .
	manualset3
162636	5	412070	7	NULL	NULL	NULL	NULL	bubble	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relationship between the volume of an intraocular gas bubble and the area of retina covered by the bubble was studied with the use of both a transparent model and a mathematical model of the vitreous cavity .
	manualset3
162637	6	412070	7	NULL	NULL	0	NULL	transparent model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between the volume of an intraocular gas bubble and the area of retina covered by the bubble was studied with the use of both a transparent model and a mathematical model of the vitreous cavity .
	manualset3
162638	7	412070	7	NULL	NULL	0	NULL	mathematical model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between the volume of an intraocular gas bubble and the area of retina covered by the bubble was studied with the use of both a transparent model and a mathematical model of the vitreous cavity .
	manualset3
162639	8	412070	7	NULL	NULL	0	NULL	 vitreous cavity	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship between the volume of an intraocular gas bubble and the area of retina covered by the bubble was studied with the use of both a transparent model and a mathematical model of the vitreous cavity .
	manualset3
162640	1	412071	7	NULL	NULL	0	NULL	neurons	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	About half of the neurons were located in the nucleus reticularis gigantocellularis ( Gi ) ; the remainder were located in surrounding ( dorsal , ventral , lateral ) regions of the MRF .
	manualset3
162641	2	412071	7	NULL	NULL	NULL	NULL	 nucleus reticularis gigantocellularis ( Gi )	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	About half of the neurons were located in the nucleus reticularis gigantocellularis ( Gi ) ; the remainder were located in surrounding ( dorsal , ventral , lateral ) regions of the MRF .
	manualset3
162642	3	412071	7	NULL	NULL	0	NULL	remainder	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	About half of the neurons were located in the nucleus reticularis gigantocellularis ( Gi ) ; the remainder were located in surrounding ( dorsal , ventral , lateral ) regions of the MRF .
	manualset3
162643	4	412071	7	NULL	NULL	0	NULL	dorsal regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	About half of the neurons were located in the nucleus reticularis gigantocellularis ( Gi ) ; the remainder were located in surrounding ( dorsal , ventral , lateral ) regions of the MRF .
	manualset3
162644	5	412071	7	NULL	NULL	0	NULL	ventral regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	About half of the neurons were located in the nucleus reticularis gigantocellularis ( Gi ) ; the remainder were located in surrounding ( dorsal , ventral , lateral ) regions of the MRF .
	manualset3
162645	6	412071	7	NULL	NULL	0	NULL	 lateral regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	About half of the neurons were located in the nucleus reticularis gigantocellularis ( Gi ) ; the remainder were located in surrounding ( dorsal , ventral , lateral ) regions of the MRF .
	manualset3
162646	7	412071	7	NULL	NULL	NULL	NULL	 MRF 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	About half of the neurons were located in the nucleus reticularis gigantocellularis ( Gi ) ; the remainder were located in surrounding ( dorsal , ventral , lateral ) regions of the MRF .
	manualset3
162647	1	412072	7	NULL	NULL	0	NULL	relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship of T cell activation to HIV entry and generation of viral DNA intermediates was studied in freshly isolated CD4 + T lymphocytes .
	manualset3
162648	2	412072	7	NULL	NULL	0	NULL	T cell activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship of T cell activation to HIV entry and generation of viral DNA intermediates was studied in freshly isolated CD4 + T lymphocytes .
	manualset3
162649	3	412072	7	NULL	NULL	0	NULL	generation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship of T cell activation to HIV entry and generation of viral DNA intermediates was studied in freshly isolated CD4 + T lymphocytes .
	manualset3
162650	4	412072	7	NULL	NULL	0	NULL	viral DNA intermediates	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship of T cell activation to HIV entry and generation of viral DNA intermediates was studied in freshly isolated CD4 + T lymphocytes .
	manualset3
162651	5	412072	7	NULL	NULL	0	NULL	freshly isolated CD4 + T lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship of T cell activation to HIV entry and generation of viral DNA intermediates was studied in freshly isolated CD4 + T lymphocytes .
	manualset3
163806	6	412072	7	NULL	NULL	NULL	NULL	HIV entry	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relationship of T cell activation to HIV entry and generation of viral DNA intermediates was studied in freshly isolated CD4 + T lymphocytes .
	manualset3
162652	1	412073	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship of altered thyroid activity to various reproductive phenomena in gilts .
	manualset3
162653	2	412073	7	NULL	NULL	0	NULL	thyroid activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship of altered thyroid activity to various reproductive phenomena in gilts .
	manualset3
162654	3	412073	7	NULL	NULL	0	NULL	reproductive phenomena	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship of altered thyroid activity to various reproductive phenomena in gilts .
	manualset3
162655	4	412073	7	NULL	NULL	0	NULL	gilts	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship of altered thyroid activity to various reproductive phenomena in gilts .
	manualset3
162656	1	412074	7	NULL	NULL	0	NULL	 relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationships among hyperuricemia , endothelial dysfunction , and cardiovascular diseases : Molecular mechanisms and clinical implications .
	manualset3
162657	2	412074	7	NULL	NULL	0	NULL	hyperuricemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationships among hyperuricemia , endothelial dysfunction , and cardiovascular diseases : Molecular mechanisms and clinical implications .
	manualset3
162658	3	412074	7	NULL	NULL	0	NULL	endothelial dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationships among hyperuricemia , endothelial dysfunction , and cardiovascular diseases : Molecular mechanisms and clinical implications .
	manualset3
162659	4	412074	7	NULL	NULL	0	NULL	cardiovascular diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationships among hyperuricemia , endothelial dysfunction , and cardiovascular diseases : Molecular mechanisms and clinical implications .
	manualset3
162660	5	412074	7	NULL	NULL	NULL	NULL	Molecular mechanisms	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relationships among hyperuricemia , endothelial dysfunction , and cardiovascular diseases : Molecular mechanisms and clinical implications .
	manualset3
162661	6	412074	7	NULL	NULL	0	NULL	clinical implications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationships among hyperuricemia , endothelial dysfunction , and cardiovascular diseases : Molecular mechanisms and clinical implications .
	manualset3
162662	1	412075	7	NULL	NULL	0	NULL	 relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationships between human papillomavirus type 16 ( HPV 16 ) viral load , HPV 16 integration status , human immunodeficiency virus type 1 ( HIV-1 ) status , and cervical cytology were studied among women enrolled in a cohort of female sex workers in Burkina Faso .
	manualset3
162663	2	412075	7	NULL	NULL	0	NULL	 human papillomavirus type 16 ( HPV 16 ) viral load	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationships between human papillomavirus type 16 ( HPV 16 ) viral load , HPV 16 integration status , human immunodeficiency virus type 1 ( HIV-1 ) status , and cervical cytology were studied among women enrolled in a cohort of female sex workers in Burkina Faso .
	manualset3
162664	3	412075	7	NULL	NULL	NULL	NULL	HPV 16 integration status	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relationships between human papillomavirus type 16 ( HPV 16 ) viral load , HPV 16 integration status , human immunodeficiency virus type 1 ( HIV-1 ) status , and cervical cytology were studied among women enrolled in a cohort of female sex workers in Burkina Faso .
	manualset3
162665	4	412075	7	NULL	NULL	0	NULL	human immunodeficiency virus type 1 ( HIV-1 ) status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationships between human papillomavirus type 16 ( HPV 16 ) viral load , HPV 16 integration status , human immunodeficiency virus type 1 ( HIV-1 ) status , and cervical cytology were studied among women enrolled in a cohort of female sex workers in Burkina Faso .
	manualset3
162666	5	412075	7	NULL	NULL	NULL	NULL	cervical cytology	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relationships between human papillomavirus type 16 ( HPV 16 ) viral load , HPV 16 integration status , human immunodeficiency virus type 1 ( HIV-1 ) status , and cervical cytology were studied among women enrolled in a cohort of female sex workers in Burkina Faso .
	manualset3
162667	6	412075	7	NULL	NULL	0	NULL	 women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationships between human papillomavirus type 16 ( HPV 16 ) viral load , HPV 16 integration status , human immunodeficiency virus type 1 ( HIV-1 ) status , and cervical cytology were studied among women enrolled in a cohort of female sex workers in Burkina Faso .
	manualset3
162668	7	412075	7	NULL	NULL	0	NULL	cohort	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationships between human papillomavirus type 16 ( HPV 16 ) viral load , HPV 16 integration status , human immunodeficiency virus type 1 ( HIV-1 ) status , and cervical cytology were studied among women enrolled in a cohort of female sex workers in Burkina Faso .
	manualset3
162669	8	412075	7	NULL	NULL	0	NULL	female sex workers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationships between human papillomavirus type 16 ( HPV 16 ) viral load , HPV 16 integration status , human immunodeficiency virus type 1 ( HIV-1 ) status , and cervical cytology were studied among women enrolled in a cohort of female sex workers in Burkina Faso .
	manualset3
162670	9	412075	7	NULL	NULL	0	NULL	Burkina Faso	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationships between human papillomavirus type 16 ( HPV 16 ) viral load , HPV 16 integration status , human immunodeficiency virus type 1 ( HIV-1 ) status , and cervical cytology were studied among women enrolled in a cohort of female sex workers in Burkina Faso .
	manualset3
162671	1	412076	7	NULL	NULL	0	NULL	relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationships of the parabola indicate that the interaction of antigen and antibody takes place according to a definite law .
	manualset3
162672	2	412076	7	NULL	NULL	0	NULL	parabola	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationships of the parabola indicate that the interaction of antigen and antibody takes place according to a definite law .
	manualset3
162673	3	412076	7	NULL	NULL	0	NULL	interaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationships of the parabola indicate that the interaction of antigen and antibody takes place according to a definite law .
	manualset3
162674	4	412076	7	NULL	NULL	NULL	NULL	antigen	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relationships of the parabola indicate that the interaction of antigen and antibody takes place according to a definite law .
	manualset3
162675	5	412076	7	NULL	NULL	0	NULL	antibody	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationships of the parabola indicate that the interaction of antigen and antibody takes place according to a definite law .
	manualset3
162676	6	412076	7	NULL	NULL	NULL	NULL	law	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relationships of the parabola indicate that the interaction of antigen and antibody takes place according to a definite law .
	manualset3
162677	1	412077	7	NULL	NULL	0	NULL	relative affinity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative affinity of various drugs for the sites labeled by ( + / - ) -3 H-lofexidine perfectly corresponded with that for the specific binding sites identified by 3H-clonidine and 3H-guanfacine .
	manualset3
162678	2	412077	7	NULL	NULL	0	NULL	drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative affinity of various drugs for the sites labeled by ( + / - ) -3 H-lofexidine perfectly corresponded with that for the specific binding sites identified by 3H-clonidine and 3H-guanfacine .
	manualset3
162679	3	412077	7	NULL	NULL	NULL	NULL	sites	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relative affinity of various drugs for the sites labeled by ( + / - ) -3 H-lofexidine perfectly corresponded with that for the specific binding sites identified by 3H-clonidine and 3H-guanfacine .
	manualset3
162680	4	412077	7	NULL	NULL	NULL	NULL	( + / - ) -3 H-lofexidine	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relative affinity of various drugs for the sites labeled by ( + / - ) -3 H-lofexidine perfectly corresponded with that for the specific binding sites identified by 3H-clonidine and 3H-guanfacine .
	manualset3
162681	5	412077	7	NULL	NULL	NULL	NULL	binding sites	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relative affinity of various drugs for the sites labeled by ( + / - ) -3 H-lofexidine perfectly corresponded with that for the specific binding sites identified by 3H-clonidine and 3H-guanfacine .
	manualset3
162682	6	412077	7	NULL	NULL	NULL	NULL	3H-clonidine	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relative affinity of various drugs for the sites labeled by ( + / - ) -3 H-lofexidine perfectly corresponded with that for the specific binding sites identified by 3H-clonidine and 3H-guanfacine .
	manualset3
162683	7	412077	7	NULL	NULL	NULL	NULL	3H-guanfacine 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relative affinity of various drugs for the sites labeled by ( + / - ) -3 H-lofexidine perfectly corresponded with that for the specific binding sites identified by 3H-clonidine and 3H-guanfacine .
	manualset3
162684	1	412078	7	NULL	NULL	0	NULL	relative potencies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative potencies in human TLR7-based primary reporter gene assays were paralleled by interferon-alpha induction activities in whole human blood models .
	manualset3
162685	2	412078	7	NULL	NULL	0	NULL	human TLR7-based primary reporter gene assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative potencies in human TLR7-based primary reporter gene assays were paralleled by interferon-alpha induction activities in whole human blood models .
	manualset3
162686	3	412078	7	NULL	NULL	0	NULL	 interferon-alpha induction activities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative potencies in human TLR7-based primary reporter gene assays were paralleled by interferon-alpha induction activities in whole human blood models .
	manualset3
162687	4	412078	7	NULL	NULL	NULL	NULL	whole human blood models	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relative potencies in human TLR7-based primary reporter gene assays were paralleled by interferon-alpha induction activities in whole human blood models .
	manualset3
162688	1	412079	7	NULL	NULL	0	NULL	Clinical utility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical utility of EC glue in retrosigmoid approach surgery ) .
	manualset3
162689	2	412079	7	NULL	NULL	0	NULL	EC glue	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical utility of EC glue in retrosigmoid approach surgery ) .
	manualset3
162690	3	412079	7	NULL	NULL	0	NULL	retrosigmoid approach surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical utility of EC glue in retrosigmoid approach surgery ) .
	manualset3
162691	1	412080	7	NULL	NULL	0	NULL	1 kR	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	About 1 kR of 5577 A was also observed , but the 5200-A emission was too low for reliable detection .
	manualset3
162692	2	412080	7	NULL	NULL	0	NULL	5577 A	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	About 1 kR of 5577 A was also observed , but the 5200-A emission was too low for reliable detection .
	manualset3
162693	3	412080	7	NULL	NULL	NULL	NULL	5200-A emission	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	About 1 kR of 5577 A was also observed , but the 5200-A emission was too low for reliable detection .
	manualset3
162694	4	412080	7	NULL	NULL	0	NULL	 reliable detection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	About 1 kR of 5577 A was also observed , but the 5200-A emission was too low for reliable detection .
	manualset3
162705	1	412081	7	NULL	NULL	0	NULL	 relative risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative risk of admission for Asian men compared with white men aged 45-64 years was 2.65 ( 95 % confidence interval 2.20 to 3.19 ) and the risk for Asian men was high for both myocardial infarction and ischemia when analyzed separately .
	manualset3
162706	2	412081	7	NULL	NULL	0	NULL	admission	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative risk of admission for Asian men compared with white men aged 45-64 years was 2.65 ( 95 % confidence interval 2.20 to 3.19 ) and the risk for Asian men was high for both myocardial infarction and ischemia when analyzed separately .
	manualset3
162707	3	412081	7	NULL	NULL	0	NULL	Asian men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative risk of admission for Asian men compared with white men aged 45-64 years was 2.65 ( 95 % confidence interval 2.20 to 3.19 ) and the risk for Asian men was high for both myocardial infarction and ischemia when analyzed separately .
	manualset3
162708	4	412081	7	NULL	NULL	0	NULL	white men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative risk of admission for Asian men compared with white men aged 45-64 years was 2.65 ( 95 % confidence interval 2.20 to 3.19 ) and the risk for Asian men was high for both myocardial infarction and ischemia when analyzed separately .
	manualset3
162709	5	412081	7	NULL	NULL	0	NULL	45-64 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative risk of admission for Asian men compared with white men aged 45-64 years was 2.65 ( 95 % confidence interval 2.20 to 3.19 ) and the risk for Asian men was high for both myocardial infarction and ischemia when analyzed separately .
	manualset3
162710	6	412081	7	NULL	NULL	0	NULL	2.65	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative risk of admission for Asian men compared with white men aged 45-64 years was 2.65 ( 95 % confidence interval 2.20 to 3.19 ) and the risk for Asian men was high for both myocardial infarction and ischemia when analyzed separately .
	manualset3
162711	7	412081	7	NULL	NULL	0	NULL	95 % confidence interval	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative risk of admission for Asian men compared with white men aged 45-64 years was 2.65 ( 95 % confidence interval 2.20 to 3.19 ) and the risk for Asian men was high for both myocardial infarction and ischemia when analyzed separately .
	manualset3
162712	8	412081	7	NULL	NULL	0	NULL	2.20 to 3.19	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative risk of admission for Asian men compared with white men aged 45-64 years was 2.65 ( 95 % confidence interval 2.20 to 3.19 ) and the risk for Asian men was high for both myocardial infarction and ischemia when analyzed separately .
	manualset3
162713	9	412081	7	NULL	NULL	0	NULL	 risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative risk of admission for Asian men compared with white men aged 45-64 years was 2.65 ( 95 % confidence interval 2.20 to 3.19 ) and the risk for Asian men was high for both myocardial infarction and ischemia when analyzed separately .
	manualset3
162714	10	412081	7	NULL	NULL	0	NULL	Asian men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative risk of admission for Asian men compared with white men aged 45-64 years was 2.65 ( 95 % confidence interval 2.20 to 3.19 ) and the risk for Asian men was high for both myocardial infarction and ischemia when analyzed separately .
	manualset3
162715	11	412081	7	NULL	NULL	0	NULL	myocardial infarction	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative risk of admission for Asian men compared with white men aged 45-64 years was 2.65 ( 95 % confidence interval 2.20 to 3.19 ) and the risk for Asian men was high for both myocardial infarction and ischemia when analyzed separately .
	manualset3
162716	12	412081	7	NULL	NULL	0	NULL	myocardial ischemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative risk of admission for Asian men compared with white men aged 45-64 years was 2.65 ( 95 % confidence interval 2.20 to 3.19 ) and the risk for Asian men was high for both myocardial infarction and ischemia when analyzed separately .
	manualset3
162717	1	412082	7	NULL	NULL	NULL	NULL	relative risks	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relative risks comparing the highest quintile of animal fat intake with the lowest were 1.42 for men ( 95 % confidence interval ( CI ) : 0.91 , 2.20 ; p for trend = 0.1 ) and 0.65 for women ( 95 % CI : 0.36 , 1.16 ; p for trend = 0.3 ) .
	manualset3
162718	2	412082	7	NULL	NULL	0	NULL	 highest quintile	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative risks comparing the highest quintile of animal fat intake with the lowest were 1.42 for men ( 95 % confidence interval ( CI ) : 0.91 , 2.20 ; p for trend = 0.1 ) and 0.65 for women ( 95 % CI : 0.36 , 1.16 ; p for trend = 0.3 ) .
	manualset3
162719	3	412082	7	NULL	NULL	NULL	NULL	animal fat intake	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relative risks comparing the highest quintile of animal fat intake with the lowest were 1.42 for men ( 95 % confidence interval ( CI ) : 0.91 , 2.20 ; p for trend = 0.1 ) and 0.65 for women ( 95 % CI : 0.36 , 1.16 ; p for trend = 0.3 ) .
	manualset3
162720	4	412082	7	NULL	NULL	0	NULL	1.42	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative risks comparing the highest quintile of animal fat intake with the lowest were 1.42 for men ( 95 % confidence interval ( CI ) : 0.91 , 2.20 ; p for trend = 0.1 ) and 0.65 for women ( 95 % CI : 0.36 , 1.16 ; p for trend = 0.3 ) .
	manualset3
162721	5	412082	7	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative risks comparing the highest quintile of animal fat intake with the lowest were 1.42 for men ( 95 % confidence interval ( CI ) : 0.91 , 2.20 ; p for trend = 0.1 ) and 0.65 for women ( 95 % CI : 0.36 , 1.16 ; p for trend = 0.3 ) .
	manualset3
162722	6	412082	7	NULL	NULL	0	NULL	95 % confidence interval ( CI ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative risks comparing the highest quintile of animal fat intake with the lowest were 1.42 for men ( 95 % confidence interval ( CI ) : 0.91 , 2.20 ; p for trend = 0.1 ) and 0.65 for women ( 95 % CI : 0.36 , 1.16 ; p for trend = 0.3 ) .
	manualset3
162723	7	412082	7	NULL	NULL	0	NULL	0.91	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative risks comparing the highest quintile of animal fat intake with the lowest were 1.42 for men ( 95 % confidence interval ( CI ) : 0.91 , 2.20 ; p for trend = 0.1 ) and 0.65 for women ( 95 % CI : 0.36 , 1.16 ; p for trend = 0.3 ) .
	manualset3
162724	8	412082	7	NULL	NULL	0	NULL	2.20	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative risks comparing the highest quintile of animal fat intake with the lowest were 1.42 for men ( 95 % confidence interval ( CI ) : 0.91 , 2.20 ; p for trend = 0.1 ) and 0.65 for women ( 95 % CI : 0.36 , 1.16 ; p for trend = 0.3 ) .
	manualset3
162725	9	412082	7	NULL	NULL	0	NULL	p for trend = 0.1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative risks comparing the highest quintile of animal fat intake with the lowest were 1.42 for men ( 95 % confidence interval ( CI ) : 0.91 , 2.20 ; p for trend = 0.1 ) and 0.65 for women ( 95 % CI : 0.36 , 1.16 ; p for trend = 0.3 ) .
	manualset3
162726	10	412082	7	NULL	NULL	0	NULL	0.65	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative risks comparing the highest quintile of animal fat intake with the lowest were 1.42 for men ( 95 % confidence interval ( CI ) : 0.91 , 2.20 ; p for trend = 0.1 ) and 0.65 for women ( 95 % CI : 0.36 , 1.16 ; p for trend = 0.3 ) .
	manualset3
162727	11	412082	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative risks comparing the highest quintile of animal fat intake with the lowest were 1.42 for men ( 95 % confidence interval ( CI ) : 0.91 , 2.20 ; p for trend = 0.1 ) and 0.65 for women ( 95 % CI : 0.36 , 1.16 ; p for trend = 0.3 ) .
	manualset3
162728	12	412082	7	NULL	NULL	0	NULL	95 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative risks comparing the highest quintile of animal fat intake with the lowest were 1.42 for men ( 95 % confidence interval ( CI ) : 0.91 , 2.20 ; p for trend = 0.1 ) and 0.65 for women ( 95 % CI : 0.36 , 1.16 ; p for trend = 0.3 ) .
	manualset3
162729	13	412082	7	NULL	NULL	0	NULL	CI : 0.36	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative risks comparing the highest quintile of animal fat intake with the lowest were 1.42 for men ( 95 % confidence interval ( CI ) : 0.91 , 2.20 ; p for trend = 0.1 ) and 0.65 for women ( 95 % CI : 0.36 , 1.16 ; p for trend = 0.3 ) .
	manualset3
162730	14	412082	7	NULL	NULL	0	NULL	1.16	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative risks comparing the highest quintile of animal fat intake with the lowest were 1.42 for men ( 95 % confidence interval ( CI ) : 0.91 , 2.20 ; p for trend = 0.1 ) and 0.65 for women ( 95 % CI : 0.36 , 1.16 ; p for trend = 0.3 ) .
	manualset3
162731	15	412082	7	NULL	NULL	0	NULL	p for trend = 0.3	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative risks comparing the highest quintile of animal fat intake with the lowest were 1.42 for men ( 95 % confidence interval ( CI ) : 0.91 , 2.20 ; p for trend = 0.1 ) and 0.65 for women ( 95 % CI : 0.36 , 1.16 ; p for trend = 0.3 ) .
	manualset3
162732	1	412083	7	NULL	NULL	0	NULL	 roles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative roles of different receptor systems in compensating for vestibular loss were studied in 18 children ( 12 to 16 years of age ) with congenital or early acquired bilateral vestibular loss ( BVL ) and impaired hearing , and compared to that in 33 normal children ( 9 to 16 years of age ) .
	manualset3
162733	2	412083	7	NULL	NULL	0	NULL	receptor systems	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative roles of different receptor systems in compensating for vestibular loss were studied in 18 children ( 12 to 16 years of age ) with congenital or early acquired bilateral vestibular loss ( BVL ) and impaired hearing , and compared to that in 33 normal children ( 9 to 16 years of age ) .
	manualset3
162734	3	412083	7	NULL	NULL	0	NULL	vestibular loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative roles of different receptor systems in compensating for vestibular loss were studied in 18 children ( 12 to 16 years of age ) with congenital or early acquired bilateral vestibular loss ( BVL ) and impaired hearing , and compared to that in 33 normal children ( 9 to 16 years of age ) .
	manualset3
162735	4	412083	7	NULL	NULL	0	NULL	18 children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative roles of different receptor systems in compensating for vestibular loss were studied in 18 children ( 12 to 16 years of age ) with congenital or early acquired bilateral vestibular loss ( BVL ) and impaired hearing , and compared to that in 33 normal children ( 9 to 16 years of age ) .
	manualset3
162736	5	412083	7	NULL	NULL	0	NULL	12 to 16 years of age	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative roles of different receptor systems in compensating for vestibular loss were studied in 18 children ( 12 to 16 years of age ) with congenital or early acquired bilateral vestibular loss ( BVL ) and impaired hearing , and compared to that in 33 normal children ( 9 to 16 years of age ) .
	manualset3
162737	6	412083	7	NULL	NULL	0	NULL	congenital or early acquired bilateral vestibular loss ( BVL )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative roles of different receptor systems in compensating for vestibular loss were studied in 18 children ( 12 to 16 years of age ) with congenital or early acquired bilateral vestibular loss ( BVL ) and impaired hearing , and compared to that in 33 normal children ( 9 to 16 years of age ) .
	manualset3
162738	7	412083	7	NULL	NULL	0	NULL	impaired hearing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative roles of different receptor systems in compensating for vestibular loss were studied in 18 children ( 12 to 16 years of age ) with congenital or early acquired bilateral vestibular loss ( BVL ) and impaired hearing , and compared to that in 33 normal children ( 9 to 16 years of age ) .
	manualset3
162739	8	412083	7	NULL	NULL	0	NULL	33 normal children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative roles of different receptor systems in compensating for vestibular loss were studied in 18 children ( 12 to 16 years of age ) with congenital or early acquired bilateral vestibular loss ( BVL ) and impaired hearing , and compared to that in 33 normal children ( 9 to 16 years of age ) .
	manualset3
162740	9	412083	7	NULL	NULL	0	NULL	9 to 16 years of age 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative roles of different receptor systems in compensating for vestibular loss were studied in 18 children ( 12 to 16 years of age ) with congenital or early acquired bilateral vestibular loss ( BVL ) and impaired hearing , and compared to that in 33 normal children ( 9 to 16 years of age ) .
	manualset3
162741	1	412084	7	NULL	NULL	0	NULL	sensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative sensitivity and specificity of ultrasonography is compared with conventional radiologic modalities .
	manualset3
162742	2	412084	7	NULL	NULL	0	NULL	specificity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative sensitivity and specificity of ultrasonography is compared with conventional radiologic modalities .
	manualset3
162743	3	412084	7	NULL	NULL	0	NULL	ultrasonography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative sensitivity and specificity of ultrasonography is compared with conventional radiologic modalities .
	manualset3
162744	4	412084	7	NULL	NULL	0	NULL	conventional radiologic modalities 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative sensitivity and specificity of ultrasonography is compared with conventional radiologic modalities .
	manualset3
162745	1	412085	7	NULL	NULL	NULL	NULL	 relative stabilization	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relative stabilization of the conformers is related to two factors : ( i ) the reduction of the electron population experienced by the hydrogens of the central methylene when they display more gauche arrangements to lone pairs ( lp ) and ( ii ) the reduction of the electron population of aminic hydrogens when the corresponding N-H bond is in a parallel arrangement to the lone pair of another N. The former depletion takes place in lp-N-C-N antiperiplanar dispositions , whereas the latter is shown in lp-N-C-N gauche arrangements .
	manualset3
162746	2	412085	7	NULL	NULL	0	NULL	conformers	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative stabilization of the conformers is related to two factors : ( i ) the reduction of the electron population experienced by the hydrogens of the central methylene when they display more gauche arrangements to lone pairs ( lp ) and ( ii ) the reduction of the electron population of aminic hydrogens when the corresponding N-H bond is in a parallel arrangement to the lone pair of another N. The former depletion takes place in lp-N-C-N antiperiplanar dispositions , whereas the latter is shown in lp-N-C-N gauche arrangements .
	manualset3
162747	3	412085	7	NULL	NULL	0	NULL	two factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative stabilization of the conformers is related to two factors : ( i ) the reduction of the electron population experienced by the hydrogens of the central methylene when they display more gauche arrangements to lone pairs ( lp ) and ( ii ) the reduction of the electron population of aminic hydrogens when the corresponding N-H bond is in a parallel arrangement to the lone pair of another N. The former depletion takes place in lp-N-C-N antiperiplanar dispositions , whereas the latter is shown in lp-N-C-N gauche arrangements .
	manualset3
162748	4	412085	7	NULL	NULL	0	NULL	reduction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative stabilization of the conformers is related to two factors : ( i ) the reduction of the electron population experienced by the hydrogens of the central methylene when they display more gauche arrangements to lone pairs ( lp ) and ( ii ) the reduction of the electron population of aminic hydrogens when the corresponding N-H bond is in a parallel arrangement to the lone pair of another N. The former depletion takes place in lp-N-C-N antiperiplanar dispositions , whereas the latter is shown in lp-N-C-N gauche arrangements .
	manualset3
162749	5	412085	7	NULL	NULL	0	NULL	electron population	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative stabilization of the conformers is related to two factors : ( i ) the reduction of the electron population experienced by the hydrogens of the central methylene when they display more gauche arrangements to lone pairs ( lp ) and ( ii ) the reduction of the electron population of aminic hydrogens when the corresponding N-H bond is in a parallel arrangement to the lone pair of another N. The former depletion takes place in lp-N-C-N antiperiplanar dispositions , whereas the latter is shown in lp-N-C-N gauche arrangements .
	manualset3
162750	6	412085	7	NULL	NULL	NULL	NULL	hydrogens 	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relative stabilization of the conformers is related to two factors : ( i ) the reduction of the electron population experienced by the hydrogens of the central methylene when they display more gauche arrangements to lone pairs ( lp ) and ( ii ) the reduction of the electron population of aminic hydrogens when the corresponding N-H bond is in a parallel arrangement to the lone pair of another N. The former depletion takes place in lp-N-C-N antiperiplanar dispositions , whereas the latter is shown in lp-N-C-N gauche arrangements .
	manualset3
162751	7	412085	7	NULL	NULL	0	NULL	central methylene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative stabilization of the conformers is related to two factors : ( i ) the reduction of the electron population experienced by the hydrogens of the central methylene when they display more gauche arrangements to lone pairs ( lp ) and ( ii ) the reduction of the electron population of aminic hydrogens when the corresponding N-H bond is in a parallel arrangement to the lone pair of another N. The former depletion takes place in lp-N-C-N antiperiplanar dispositions , whereas the latter is shown in lp-N-C-N gauche arrangements .
	manualset3
162752	8	412085	7	NULL	NULL	0	NULL	gauche arrangements	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative stabilization of the conformers is related to two factors : ( i ) the reduction of the electron population experienced by the hydrogens of the central methylene when they display more gauche arrangements to lone pairs ( lp ) and ( ii ) the reduction of the electron population of aminic hydrogens when the corresponding N-H bond is in a parallel arrangement to the lone pair of another N. The former depletion takes place in lp-N-C-N antiperiplanar dispositions , whereas the latter is shown in lp-N-C-N gauche arrangements .
	manualset3
162753	9	412085	7	NULL	NULL	0	NULL	 lone pairs ( lp )	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative stabilization of the conformers is related to two factors : ( i ) the reduction of the electron population experienced by the hydrogens of the central methylene when they display more gauche arrangements to lone pairs ( lp ) and ( ii ) the reduction of the electron population of aminic hydrogens when the corresponding N-H bond is in a parallel arrangement to the lone pair of another N. The former depletion takes place in lp-N-C-N antiperiplanar dispositions , whereas the latter is shown in lp-N-C-N gauche arrangements .
	manualset3
162754	10	412085	7	NULL	NULL	0	NULL	reduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative stabilization of the conformers is related to two factors : ( i ) the reduction of the electron population experienced by the hydrogens of the central methylene when they display more gauche arrangements to lone pairs ( lp ) and ( ii ) the reduction of the electron population of aminic hydrogens when the corresponding N-H bond is in a parallel arrangement to the lone pair of another N. The former depletion takes place in lp-N-C-N antiperiplanar dispositions , whereas the latter is shown in lp-N-C-N gauche arrangements .
	manualset3
162755	11	412085	7	NULL	NULL	0	NULL	electron population	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative stabilization of the conformers is related to two factors : ( i ) the reduction of the electron population experienced by the hydrogens of the central methylene when they display more gauche arrangements to lone pairs ( lp ) and ( ii ) the reduction of the electron population of aminic hydrogens when the corresponding N-H bond is in a parallel arrangement to the lone pair of another N. The former depletion takes place in lp-N-C-N antiperiplanar dispositions , whereas the latter is shown in lp-N-C-N gauche arrangements .
	manualset3
162756	12	412085	7	NULL	NULL	NULL	NULL	aminic hydrogens	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relative stabilization of the conformers is related to two factors : ( i ) the reduction of the electron population experienced by the hydrogens of the central methylene when they display more gauche arrangements to lone pairs ( lp ) and ( ii ) the reduction of the electron population of aminic hydrogens when the corresponding N-H bond is in a parallel arrangement to the lone pair of another N. The former depletion takes place in lp-N-C-N antiperiplanar dispositions , whereas the latter is shown in lp-N-C-N gauche arrangements .
	manualset3
162757	13	412085	7	NULL	NULL	0	NULL	N-H bond	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative stabilization of the conformers is related to two factors : ( i ) the reduction of the electron population experienced by the hydrogens of the central methylene when they display more gauche arrangements to lone pairs ( lp ) and ( ii ) the reduction of the electron population of aminic hydrogens when the corresponding N-H bond is in a parallel arrangement to the lone pair of another N. The former depletion takes place in lp-N-C-N antiperiplanar dispositions , whereas the latter is shown in lp-N-C-N gauche arrangements .
	manualset3
162758	14	412085	7	NULL	NULL	0	NULL	parallel arrangement	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative stabilization of the conformers is related to two factors : ( i ) the reduction of the electron population experienced by the hydrogens of the central methylene when they display more gauche arrangements to lone pairs ( lp ) and ( ii ) the reduction of the electron population of aminic hydrogens when the corresponding N-H bond is in a parallel arrangement to the lone pair of another N. The former depletion takes place in lp-N-C-N antiperiplanar dispositions , whereas the latter is shown in lp-N-C-N gauche arrangements .
	manualset3
162759	15	412085	7	NULL	NULL	0	NULL	lone pair	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative stabilization of the conformers is related to two factors : ( i ) the reduction of the electron population experienced by the hydrogens of the central methylene when they display more gauche arrangements to lone pairs ( lp ) and ( ii ) the reduction of the electron population of aminic hydrogens when the corresponding N-H bond is in a parallel arrangement to the lone pair of another N. The former depletion takes place in lp-N-C-N antiperiplanar dispositions , whereas the latter is shown in lp-N-C-N gauche arrangements .
	manualset3
162760	16	412085	7	NULL	NULL	0	NULL	N	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative stabilization of the conformers is related to two factors : ( i ) the reduction of the electron population experienced by the hydrogens of the central methylene when they display more gauche arrangements to lone pairs ( lp ) and ( ii ) the reduction of the electron population of aminic hydrogens when the corresponding N-H bond is in a parallel arrangement to the lone pair of another N. The former depletion takes place in lp-N-C-N antiperiplanar dispositions , whereas the latter is shown in lp-N-C-N gauche arrangements .
	manualset3
162761	17	412085	7	NULL	NULL	0	NULL	former depletion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative stabilization of the conformers is related to two factors : ( i ) the reduction of the electron population experienced by the hydrogens of the central methylene when they display more gauche arrangements to lone pairs ( lp ) and ( ii ) the reduction of the electron population of aminic hydrogens when the corresponding N-H bond is in a parallel arrangement to the lone pair of another N. The former depletion takes place in lp-N-C-N antiperiplanar dispositions , whereas the latter is shown in lp-N-C-N gauche arrangements .
	manualset3
162762	18	412085	7	NULL	NULL	0	NULL	 lp-N-C-N antiperiplanar dispositions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative stabilization of the conformers is related to two factors : ( i ) the reduction of the electron population experienced by the hydrogens of the central methylene when they display more gauche arrangements to lone pairs ( lp ) and ( ii ) the reduction of the electron population of aminic hydrogens when the corresponding N-H bond is in a parallel arrangement to the lone pair of another N. The former depletion takes place in lp-N-C-N antiperiplanar dispositions , whereas the latter is shown in lp-N-C-N gauche arrangements .
	manualset3
162763	19	412085	7	NULL	NULL	0	NULL	lp-N-C-N gauche arrangements	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative stabilization of the conformers is related to two factors : ( i ) the reduction of the electron population experienced by the hydrogens of the central methylene when they display more gauche arrangements to lone pairs ( lp ) and ( ii ) the reduction of the electron population of aminic hydrogens when the corresponding N-H bond is in a parallel arrangement to the lone pair of another N. The former depletion takes place in lp-N-C-N antiperiplanar dispositions , whereas the latter is shown in lp-N-C-N gauche arrangements .
	manualset3
162764	1	412086	7	NULL	NULL	0	NULL	relative standard uncertainty	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative standard uncertainty computed for aflatoxin B ( 1 ) was 16.3 % .
	manualset3
162765	2	412086	7	NULL	NULL	0	NULL	aflatoxin B ( 1 )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative standard uncertainty computed for aflatoxin B ( 1 ) was 16.3 % .
	manualset3
162766	3	412086	7	NULL	NULL	0	NULL	16.3 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative standard uncertainty computed for aflatoxin B ( 1 ) was 16.3 % .
	manualset3
162767	1	412087	7	NULL	NULL	0	NULL	underperfusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative underperfusion of active skeletal muscle in heart failure may tonically activate the metaboreflex and this probably contributes to the enhanced sympatho-excitation seen during exercise in heart failure .
	manualset3
162768	2	412087	7	NULL	NULL	0	NULL	active skeletal muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative underperfusion of active skeletal muscle in heart failure may tonically activate the metaboreflex and this probably contributes to the enhanced sympatho-excitation seen during exercise in heart failure .
	manualset3
162769	3	412087	7	NULL	NULL	0	NULL	heart failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative underperfusion of active skeletal muscle in heart failure may tonically activate the metaboreflex and this probably contributes to the enhanced sympatho-excitation seen during exercise in heart failure .
	manualset3
162770	4	412087	7	NULL	NULL	0	NULL	metaboreflex	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative underperfusion of active skeletal muscle in heart failure may tonically activate the metaboreflex and this probably contributes to the enhanced sympatho-excitation seen during exercise in heart failure .
	manualset3
162771	5	412087	7	NULL	NULL	0	NULL	enhanced sympatho-excitation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative underperfusion of active skeletal muscle in heart failure may tonically activate the metaboreflex and this probably contributes to the enhanced sympatho-excitation seen during exercise in heart failure .
	manualset3
162772	6	412087	7	NULL	NULL	0	NULL	exercise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative underperfusion of active skeletal muscle in heart failure may tonically activate the metaboreflex and this probably contributes to the enhanced sympatho-excitation seen during exercise in heart failure .
	manualset3
162773	7	412087	7	NULL	NULL	0	NULL	heart failure 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative underperfusion of active skeletal muscle in heart failure may tonically activate the metaboreflex and this probably contributes to the enhanced sympatho-excitation seen during exercise in heart failure .
	manualset3
162774	1	412088	7	NULL	NULL	0	NULL	late appearance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The relatively late appearance of SIF cells in the sphenopalatine ganglion argues against the hypothesis that SIF cells are the precursors of all autonomic neurons .
	manualset3
162775	2	412088	7	NULL	NULL	0	NULL	SIF cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The relatively late appearance of SIF cells in the sphenopalatine ganglion argues against the hypothesis that SIF cells are the precursors of all autonomic neurons .
	manualset3
162776	3	412088	7	NULL	NULL	0	NULL	 sphenopalatine ganglion	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The relatively late appearance of SIF cells in the sphenopalatine ganglion argues against the hypothesis that SIF cells are the precursors of all autonomic neurons .
	manualset3
162777	4	412088	7	NULL	NULL	0	NULL	hypothesis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The relatively late appearance of SIF cells in the sphenopalatine ganglion argues against the hypothesis that SIF cells are the precursors of all autonomic neurons .
	manualset3
162778	5	412088	7	NULL	NULL	0	NULL	SIF cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The relatively late appearance of SIF cells in the sphenopalatine ganglion argues against the hypothesis that SIF cells are the precursors of all autonomic neurons .
	manualset3
162779	6	412088	7	NULL	NULL	0	NULL	precursors	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The relatively late appearance of SIF cells in the sphenopalatine ganglion argues against the hypothesis that SIF cells are the precursors of all autonomic neurons .
	manualset3
162780	7	412088	7	NULL	NULL	0	NULL	autonomic neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The relatively late appearance of SIF cells in the sphenopalatine ganglion argues against the hypothesis that SIF cells are the precursors of all autonomic neurons .
	manualset3
162781	1	412089	7	NULL	NULL	0	NULL	16S rRNA gene sequence similarity	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The relatively low 16S rRNA gene sequence similarity of 96.0 % to C. lactis M 2040 ( T ) and marked differences in the polar lipid profiles as well as the results of physiological tests and the DNA-DNA hybridization data support the creation of a novel species , for which the name Camelimonas abortus sp .
	manualset3
162782	2	412089	7	NULL	NULL	0	NULL	 96.0 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The relatively low 16S rRNA gene sequence similarity of 96.0 % to C. lactis M 2040 ( T ) and marked differences in the polar lipid profiles as well as the results of physiological tests and the DNA-DNA hybridization data support the creation of a novel species , for which the name Camelimonas abortus sp .
	manualset3
162783	3	412089	7	NULL	NULL	0	NULL	C. lactis M 2040 ( T )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The relatively low 16S rRNA gene sequence similarity of 96.0 % to C. lactis M 2040 ( T ) and marked differences in the polar lipid profiles as well as the results of physiological tests and the DNA-DNA hybridization data support the creation of a novel species , for which the name Camelimonas abortus sp .
	manualset3
162784	4	412089	7	NULL	NULL	0	NULL	polar lipid profiles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The relatively low 16S rRNA gene sequence similarity of 96.0 % to C. lactis M 2040 ( T ) and marked differences in the polar lipid profiles as well as the results of physiological tests and the DNA-DNA hybridization data support the creation of a novel species , for which the name Camelimonas abortus sp .
	manualset3
162785	5	412089	7	NULL	NULL	0	NULL	 results 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The relatively low 16S rRNA gene sequence similarity of 96.0 % to C. lactis M 2040 ( T ) and marked differences in the polar lipid profiles as well as the results of physiological tests and the DNA-DNA hybridization data support the creation of a novel species , for which the name Camelimonas abortus sp .
	manualset3
162786	6	412089	7	NULL	NULL	0	NULL	physiological tests	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The relatively low 16S rRNA gene sequence similarity of 96.0 % to C. lactis M 2040 ( T ) and marked differences in the polar lipid profiles as well as the results of physiological tests and the DNA-DNA hybridization data support the creation of a novel species , for which the name Camelimonas abortus sp .
	manualset3
162787	7	412089	7	NULL	NULL	0	NULL	DNA-DNA hybridization data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The relatively low 16S rRNA gene sequence similarity of 96.0 % to C. lactis M 2040 ( T ) and marked differences in the polar lipid profiles as well as the results of physiological tests and the DNA-DNA hybridization data support the creation of a novel species , for which the name Camelimonas abortus sp .
	manualset3
162788	8	412089	7	NULL	NULL	0	NULL	creation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The relatively low 16S rRNA gene sequence similarity of 96.0 % to C. lactis M 2040 ( T ) and marked differences in the polar lipid profiles as well as the results of physiological tests and the DNA-DNA hybridization data support the creation of a novel species , for which the name Camelimonas abortus sp .
	manualset3
162789	9	412089	7	NULL	NULL	0	NULL	novel species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The relatively low 16S rRNA gene sequence similarity of 96.0 % to C. lactis M 2040 ( T ) and marked differences in the polar lipid profiles as well as the results of physiological tests and the DNA-DNA hybridization data support the creation of a novel species , for which the name Camelimonas abortus sp .
	manualset3
162790	10	412089	7	NULL	NULL	0	NULL	name	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The relatively low 16S rRNA gene sequence similarity of 96.0 % to C. lactis M 2040 ( T ) and marked differences in the polar lipid profiles as well as the results of physiological tests and the DNA-DNA hybridization data support the creation of a novel species , for which the name Camelimonas abortus sp .
	manualset3
162791	11	412089	7	NULL	NULL	0	NULL	Camelimonas abortus sp .	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The relatively low 16S rRNA gene sequence similarity of 96.0 % to C. lactis M 2040 ( T ) and marked differences in the polar lipid profiles as well as the results of physiological tests and the DNA-DNA hybridization data support the creation of a novel species , for which the name Camelimonas abortus sp .
	manualset3
162792	1	412090	7	NULL	NULL	NULL	NULL	relatively modest specificity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relatively modest specificity in the binding of aminoglycoside described above is to be contrasted to the subnanomolar affinities and specificity of aminoglycoside binding found using in vitro selected RNA molecules ( Wang et al. , 1996 ) .
	manualset3
162793	2	412090	7	NULL	NULL	NULL	NULL	binding	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relatively modest specificity in the binding of aminoglycoside described above is to be contrasted to the subnanomolar affinities and specificity of aminoglycoside binding found using in vitro selected RNA molecules ( Wang et al. , 1996 ) .
	manualset3
162794	3	412090	7	NULL	NULL	0	NULL	aminoglycoside	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The relatively modest specificity in the binding of aminoglycoside described above is to be contrasted to the subnanomolar affinities and specificity of aminoglycoside binding found using in vitro selected RNA molecules ( Wang et al. , 1996 ) .
	manualset3
162795	4	412090	7	NULL	NULL	0	NULL	subnanomolar affinities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relatively modest specificity in the binding of aminoglycoside described above is to be contrasted to the subnanomolar affinities and specificity of aminoglycoside binding found using in vitro selected RNA molecules ( Wang et al. , 1996 ) .
	manualset3
162796	5	412090	7	NULL	NULL	0	NULL	specificity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relatively modest specificity in the binding of aminoglycoside described above is to be contrasted to the subnanomolar affinities and specificity of aminoglycoside binding found using in vitro selected RNA molecules ( Wang et al. , 1996 ) .
	manualset3
162797	6	412090	7	NULL	NULL	0	NULL	aminoglycoside binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relatively modest specificity in the binding of aminoglycoside described above is to be contrasted to the subnanomolar affinities and specificity of aminoglycoside binding found using in vitro selected RNA molecules ( Wang et al. , 1996 ) .
	manualset3
162798	7	412090	7	NULL	NULL	0	NULL	RNA molecules	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The relatively modest specificity in the binding of aminoglycoside described above is to be contrasted to the subnanomolar affinities and specificity of aminoglycoside binding found using in vitro selected RNA molecules ( Wang et al. , 1996 ) .
	manualset3
162799	8	412090	7	NULL	NULL	0	NULL	Wang et al. ,	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	The relatively modest specificity in the binding of aminoglycoside described above is to be contrasted to the subnanomolar affinities and specificity of aminoglycoside binding found using in vitro selected RNA molecules ( Wang et al. , 1996 ) .
	manualset3
162800	9	412090	7	NULL	NULL	NULL	NULL	1996	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relatively modest specificity in the binding of aminoglycoside described above is to be contrasted to the subnanomolar affinities and specificity of aminoglycoside binding found using in vitro selected RNA molecules ( Wang et al. , 1996 ) .
	manualset3
162801	1	412091	7	NULL	NULL	0	NULL	 30 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	About 30 % of breast cancers , however , are hormone - independent because of lack of ER expression .
	manualset3
162802	2	412091	7	NULL	NULL	0	NULL	 breast cancers	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	About 30 % of breast cancers , however , are hormone - independent because of lack of ER expression .
	manualset3
162803	3	412091	7	NULL	NULL	0	NULL	 hormone - independent	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	About 30 % of breast cancers , however , are hormone - independent because of lack of ER expression .
	manualset3
162804	4	412091	7	NULL	NULL	0	NULL	 lack 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	About 30 % of breast cancers , however , are hormone - independent because of lack of ER expression .
	manualset3
162805	5	412091	7	NULL	NULL	NULL	NULL	ER expression	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	About 30 % of breast cancers , however , are hormone - independent because of lack of ER expression .
	manualset3
162806	1	412092	7	NULL	NULL	0	NULL	relaxant responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relaxant responses to acetylcholine were decreased in aortas from arthritic rats , whereas the responses to sodiumnitroprusside were not significantly different when compared to the aortas from control rats .
	manualset3
162807	2	412092	7	NULL	NULL	0	NULL	acetylcholine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The relaxant responses to acetylcholine were decreased in aortas from arthritic rats , whereas the responses to sodiumnitroprusside were not significantly different when compared to the aortas from control rats .
	manualset3
162808	3	412092	7	NULL	NULL	0	NULL	aortas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The relaxant responses to acetylcholine were decreased in aortas from arthritic rats , whereas the responses to sodiumnitroprusside were not significantly different when compared to the aortas from control rats .
	manualset3
162809	4	412092	7	NULL	NULL	0	NULL	arthritic rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The relaxant responses to acetylcholine were decreased in aortas from arthritic rats , whereas the responses to sodiumnitroprusside were not significantly different when compared to the aortas from control rats .
	manualset3
162810	5	412092	7	NULL	NULL	0	NULL	 responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relaxant responses to acetylcholine were decreased in aortas from arthritic rats , whereas the responses to sodiumnitroprusside were not significantly different when compared to the aortas from control rats .
	manualset3
162811	6	412092	7	NULL	NULL	0	NULL	sodiumnitroprusside	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The relaxant responses to acetylcholine were decreased in aortas from arthritic rats , whereas the responses to sodiumnitroprusside were not significantly different when compared to the aortas from control rats .
	manualset3
162812	7	412092	7	NULL	NULL	0	NULL	aortas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The relaxant responses to acetylcholine were decreased in aortas from arthritic rats , whereas the responses to sodiumnitroprusside were not significantly different when compared to the aortas from control rats .
	manualset3
162813	8	412092	7	NULL	NULL	0	NULL	control rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The relaxant responses to acetylcholine were decreased in aortas from arthritic rats , whereas the responses to sodiumnitroprusside were not significantly different when compared to the aortas from control rats .
	manualset3
162814	1	412093	7	NULL	NULL	0	NULL	relaxation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relaxation induced by testosterone was significantly reduced by denudation of endothelium in SHR but not WKY .
	manualset3
162815	2	412093	7	NULL	NULL	0	NULL	testosterone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The relaxation induced by testosterone was significantly reduced by denudation of endothelium in SHR but not WKY .
	manualset3
162816	3	412093	7	NULL	NULL	0	NULL	denudation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The relaxation induced by testosterone was significantly reduced by denudation of endothelium in SHR but not WKY .
	manualset3
162817	4	412093	7	NULL	NULL	0	NULL	endothelium	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The relaxation induced by testosterone was significantly reduced by denudation of endothelium in SHR but not WKY .
	manualset3
162818	5	412093	7	NULL	NULL	0	NULL	SHR	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The relaxation induced by testosterone was significantly reduced by denudation of endothelium in SHR but not WKY .
	manualset3
162819	6	412093	7	NULL	NULL	0	NULL	WKY	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The relaxation induced by testosterone was significantly reduced by denudation of endothelium in SHR but not WKY .
	manualset3
162820	1	412094	7	NULL	NULL	0	NULL	release rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The release rate of ampicillin is increased by encapsulation in neutral and negatively charged SVs and the permeation rate was slowed by dispersion of drug-loaded SVs in gellan solution .
	manualset3
162821	2	412094	7	NULL	NULL	0	NULL	ampicillin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The release rate of ampicillin is increased by encapsulation in neutral and negatively charged SVs and the permeation rate was slowed by dispersion of drug-loaded SVs in gellan solution .
	manualset3
162822	3	412094	7	NULL	NULL	0	NULL	 encapsulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The release rate of ampicillin is increased by encapsulation in neutral and negatively charged SVs and the permeation rate was slowed by dispersion of drug-loaded SVs in gellan solution .
	manualset3
162823	4	412094	7	NULL	NULL	0	NULL	neutral and negatively charged SVs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The release rate of ampicillin is increased by encapsulation in neutral and negatively charged SVs and the permeation rate was slowed by dispersion of drug-loaded SVs in gellan solution .
	manualset3
162824	5	412094	7	NULL	NULL	0	NULL	permeation rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The release rate of ampicillin is increased by encapsulation in neutral and negatively charged SVs and the permeation rate was slowed by dispersion of drug-loaded SVs in gellan solution .
	manualset3
162825	6	412094	7	NULL	NULL	NULL	NULL	dispersion	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The release rate of ampicillin is increased by encapsulation in neutral and negatively charged SVs and the permeation rate was slowed by dispersion of drug-loaded SVs in gellan solution .
	manualset3
162826	7	412094	7	NULL	NULL	0	NULL	drug-loaded SVs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The release rate of ampicillin is increased by encapsulation in neutral and negatively charged SVs and the permeation rate was slowed by dispersion of drug-loaded SVs in gellan solution .
	manualset3
162827	8	412094	7	NULL	NULL	0	NULL	gellan solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The release rate of ampicillin is increased by encapsulation in neutral and negatively charged SVs and the permeation rate was slowed by dispersion of drug-loaded SVs in gellan solution .
	manualset3
162828	1	412095	7	NULL	NULL	0	NULL	relevance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The relevance of CAM to health disparities is also discussed .
	manualset3
162829	2	412095	7	NULL	NULL	NULL	NULL	 CAM	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relevance of CAM to health disparities is also discussed .
	manualset3
162830	3	412095	7	NULL	NULL	NULL	NULL	 health disparities	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The relevance of CAM to health disparities is also discussed .
	manualset3
162831	1	412096	7	NULL	NULL	NULL	NULL	 criteria	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reliable criteria for predicting the tumor behavior are still lacking .
	manualset3
162832	3	412096	7	NULL	NULL	NULL	NULL	tumor behavior	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reliable criteria for predicting the tumor behavior are still lacking .
	manualset3
164155	2	412096	7	NULL	NULL	0	NULL	predicting	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The reliable criteria for predicting the tumor behavior are still lacking .
	manualset3
162833	1	412097	7	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The remaining patients continue to be asymptomatic to date , with platelet counts greater than 100 , 000 / cu mm .
	manualset3
162834	2	412097	7	NULL	NULL	0	NULL	date	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The remaining patients continue to be asymptomatic to date , with platelet counts greater than 100 , 000 / cu mm .
	manualset3
162835	3	412097	7	NULL	NULL	0	NULL	platelet counts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The remaining patients continue to be asymptomatic to date , with platelet counts greater than 100 , 000 / cu mm .
	manualset3
162836	4	412097	7	NULL	NULL	0	NULL	100 , 000 / cu mm 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The remaining patients continue to be asymptomatic to date , with platelet counts greater than 100 , 000 / cu mm .
	manualset3
162837	1	412098	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The remaining rats in each group underwent indocyanine green test , serologic examination , or measurement of prothrombin time .
	manualset3
162838	2	412098	7	NULL	NULL	0	NULL	group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The remaining rats in each group underwent indocyanine green test , serologic examination , or measurement of prothrombin time .
	manualset3
162839	3	412098	7	NULL	NULL	0	NULL	indocyanine green test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The remaining rats in each group underwent indocyanine green test , serologic examination , or measurement of prothrombin time .
	manualset3
162840	4	412098	7	NULL	NULL	0	NULL	serologic examination 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The remaining rats in each group underwent indocyanine green test , serologic examination , or measurement of prothrombin time .
	manualset3
162841	5	412098	7	NULL	NULL	0	NULL	measurement	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The remaining rats in each group underwent indocyanine green test , serologic examination , or measurement of prothrombin time .
	manualset3
162842	6	412098	7	NULL	NULL	0	NULL	prothrombin time	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The remaining rats in each group underwent indocyanine green test , serologic examination , or measurement of prothrombin time .
	manualset3
162843	1	412099	7	NULL	NULL	0	NULL	incomplete recovery	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The remarkable but incomplete recovery of dexterity over a period of 6-12 months , therefore , must be achieved by 1 ) optimizing the transmission of information from the cortex to the spinal cord by the substantially reduced populations of corticospinal neurons and corticobulbospinal projections and/or 2 ) the effective use of spinal circuitry in regulating the more stereotyped elements of the manual task .
	manualset3
162844	2	412099	7	NULL	NULL	0	NULL	dexterity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The remarkable but incomplete recovery of dexterity over a period of 6-12 months , therefore , must be achieved by 1 ) optimizing the transmission of information from the cortex to the spinal cord by the substantially reduced populations of corticospinal neurons and corticobulbospinal projections and/or 2 ) the effective use of spinal circuitry in regulating the more stereotyped elements of the manual task .
	manualset3
162845	3	412099	7	NULL	NULL	0	NULL	period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The remarkable but incomplete recovery of dexterity over a period of 6-12 months , therefore , must be achieved by 1 ) optimizing the transmission of information from the cortex to the spinal cord by the substantially reduced populations of corticospinal neurons and corticobulbospinal projections and/or 2 ) the effective use of spinal circuitry in regulating the more stereotyped elements of the manual task .
	manualset3
162846	4	412099	7	NULL	NULL	0	NULL	6-12 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The remarkable but incomplete recovery of dexterity over a period of 6-12 months , therefore , must be achieved by 1 ) optimizing the transmission of information from the cortex to the spinal cord by the substantially reduced populations of corticospinal neurons and corticobulbospinal projections and/or 2 ) the effective use of spinal circuitry in regulating the more stereotyped elements of the manual task .
	manualset3
162847	5	412099	7	NULL	NULL	0	NULL	 transmission	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The remarkable but incomplete recovery of dexterity over a period of 6-12 months , therefore , must be achieved by 1 ) optimizing the transmission of information from the cortex to the spinal cord by the substantially reduced populations of corticospinal neurons and corticobulbospinal projections and/or 2 ) the effective use of spinal circuitry in regulating the more stereotyped elements of the manual task .
	manualset3
162848	6	412099	7	NULL	NULL	0	NULL	information	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The remarkable but incomplete recovery of dexterity over a period of 6-12 months , therefore , must be achieved by 1 ) optimizing the transmission of information from the cortex to the spinal cord by the substantially reduced populations of corticospinal neurons and corticobulbospinal projections and/or 2 ) the effective use of spinal circuitry in regulating the more stereotyped elements of the manual task .
	manualset3
162849	7	412099	7	NULL	NULL	0	NULL	 cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The remarkable but incomplete recovery of dexterity over a period of 6-12 months , therefore , must be achieved by 1 ) optimizing the transmission of information from the cortex to the spinal cord by the substantially reduced populations of corticospinal neurons and corticobulbospinal projections and/or 2 ) the effective use of spinal circuitry in regulating the more stereotyped elements of the manual task .
	manualset3
162850	8	412099	7	NULL	NULL	0	NULL	spinal cord	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The remarkable but incomplete recovery of dexterity over a period of 6-12 months , therefore , must be achieved by 1 ) optimizing the transmission of information from the cortex to the spinal cord by the substantially reduced populations of corticospinal neurons and corticobulbospinal projections and/or 2 ) the effective use of spinal circuitry in regulating the more stereotyped elements of the manual task .
	manualset3
162851	9	412099	7	NULL	NULL	0	NULL	substantially reduced populations	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The remarkable but incomplete recovery of dexterity over a period of 6-12 months , therefore , must be achieved by 1 ) optimizing the transmission of information from the cortex to the spinal cord by the substantially reduced populations of corticospinal neurons and corticobulbospinal projections and/or 2 ) the effective use of spinal circuitry in regulating the more stereotyped elements of the manual task .
	manualset3
162852	10	412099	7	NULL	NULL	0	NULL	corticospinal neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The remarkable but incomplete recovery of dexterity over a period of 6-12 months , therefore , must be achieved by 1 ) optimizing the transmission of information from the cortex to the spinal cord by the substantially reduced populations of corticospinal neurons and corticobulbospinal projections and/or 2 ) the effective use of spinal circuitry in regulating the more stereotyped elements of the manual task .
	manualset3
162853	11	412099	7	NULL	NULL	0	NULL	corticobulbospinal projections	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The remarkable but incomplete recovery of dexterity over a period of 6-12 months , therefore , must be achieved by 1 ) optimizing the transmission of information from the cortex to the spinal cord by the substantially reduced populations of corticospinal neurons and corticobulbospinal projections and/or 2 ) the effective use of spinal circuitry in regulating the more stereotyped elements of the manual task .
	manualset3
162854	12	412099	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The remarkable but incomplete recovery of dexterity over a period of 6-12 months , therefore , must be achieved by 1 ) optimizing the transmission of information from the cortex to the spinal cord by the substantially reduced populations of corticospinal neurons and corticobulbospinal projections and/or 2 ) the effective use of spinal circuitry in regulating the more stereotyped elements of the manual task .
	manualset3
162855	13	412099	7	NULL	NULL	0	NULL	spinal circuitry	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The remarkable but incomplete recovery of dexterity over a period of 6-12 months , therefore , must be achieved by 1 ) optimizing the transmission of information from the cortex to the spinal cord by the substantially reduced populations of corticospinal neurons and corticobulbospinal projections and/or 2 ) the effective use of spinal circuitry in regulating the more stereotyped elements of the manual task .
	manualset3
162856	14	412099	7	NULL	NULL	0	NULL	stereotyped elements	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The remarkable but incomplete recovery of dexterity over a period of 6-12 months , therefore , must be achieved by 1 ) optimizing the transmission of information from the cortex to the spinal cord by the substantially reduced populations of corticospinal neurons and corticobulbospinal projections and/or 2 ) the effective use of spinal circuitry in regulating the more stereotyped elements of the manual task .
	manualset3
162857	15	412099	7	NULL	NULL	0	NULL	 manual task	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The remarkable but incomplete recovery of dexterity over a period of 6-12 months , therefore , must be achieved by 1 ) optimizing the transmission of information from the cortex to the spinal cord by the substantially reduced populations of corticospinal neurons and corticobulbospinal projections and/or 2 ) the effective use of spinal circuitry in regulating the more stereotyped elements of the manual task .
	manualset3
162858	1	412100	7	NULL	NULL	0	NULL	removal	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The removal of ineffective parts from the OspA antigen may reduce side effects and lead to a safer vaccine .
	manualset3
162859	2	412100	7	NULL	NULL	0	NULL	 ineffective parts	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The removal of ineffective parts from the OspA antigen may reduce side effects and lead to a safer vaccine .
	manualset3
162860	4	412100	7	NULL	NULL	NULL	NULL	side effects	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The removal of ineffective parts from the OspA antigen may reduce side effects and lead to a safer vaccine .
	manualset3
162861	5	412100	7	NULL	NULL	NULL	NULL	 vaccine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The removal of ineffective parts from the OspA antigen may reduce side effects and lead to a safer vaccine .
	manualset3
162862	3	412100	7	NULL	NULL	0	NULL	OspA antigen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The removal of ineffective parts from the OspA antigen may reduce side effects and lead to a safer vaccine .
	manualset3
162863	1	412101	7	NULL	NULL	0	NULL	renal involvement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The renal involvement reported in MS is believed to occur as a side effect of nephrotoxic drugs or neurogenic bladder .
	manualset3
162864	2	412101	7	NULL	NULL	0	NULL	MS 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The renal involvement reported in MS is believed to occur as a side effect of nephrotoxic drugs or neurogenic bladder .
	manualset3
162865	3	412101	7	NULL	NULL	0	NULL	side effect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The renal involvement reported in MS is believed to occur as a side effect of nephrotoxic drugs or neurogenic bladder .
	manualset3
162866	4	412101	7	NULL	NULL	0	NULL	nephrotoxic drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The renal involvement reported in MS is believed to occur as a side effect of nephrotoxic drugs or neurogenic bladder .
	manualset3
162867	5	412101	7	NULL	NULL	0	NULL	neurogenic bladder	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The renal involvement reported in MS is believed to occur as a side effect of nephrotoxic drugs or neurogenic bladder .
	manualset3
162868	1	412102	7	NULL	NULL	0	NULL	 renatured antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The renatured antibody bound 1.6 mol of digoxin per mol and had an association constant of 1.6 x 10 ( 8 ) M ( -1 ) .
	manualset3
162869	2	412102	7	NULL	NULL	0	NULL	1.6 mol	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The renatured antibody bound 1.6 mol of digoxin per mol and had an association constant of 1.6 x 10 ( 8 ) M ( -1 ) .
	manualset3
162870	3	412102	7	NULL	NULL	0	NULL	digoxin per mol 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The renatured antibody bound 1.6 mol of digoxin per mol and had an association constant of 1.6 x 10 ( 8 ) M ( -1 ) .
	manualset3
162871	4	412102	7	NULL	NULL	0	NULL	association constant	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The renatured antibody bound 1.6 mol of digoxin per mol and had an association constant of 1.6 x 10 ( 8 ) M ( -1 ) .
	manualset3
162872	5	412102	7	NULL	NULL	0	NULL	1.6 x 10 ( 8 ) M ( -1 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The renatured antibody bound 1.6 mol of digoxin per mol and had an association constant of 1.6 x 10 ( 8 ) M ( -1 ) .
	manualset3
162873	1	412103	7	NULL	NULL	0	NULL	repair	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The repair of abdominal wall defects is one of the most commonly performed general surgical procedures , with over 1 million polypropylene implants inserted each year .
	manualset3
162874	2	412103	7	NULL	NULL	0	NULL	abdominal wall defects	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The repair of abdominal wall defects is one of the most commonly performed general surgical procedures , with over 1 million polypropylene implants inserted each year .
	manualset3
162875	3	412103	7	NULL	NULL	0	NULL	general surgical procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The repair of abdominal wall defects is one of the most commonly performed general surgical procedures , with over 1 million polypropylene implants inserted each year .
	manualset3
162876	4	412103	7	NULL	NULL	0	NULL	1 million 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The repair of abdominal wall defects is one of the most commonly performed general surgical procedures , with over 1 million polypropylene implants inserted each year .
	manualset3
162877	5	412103	7	NULL	NULL	0	NULL	polypropylene implants	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The repair of abdominal wall defects is one of the most commonly performed general surgical procedures , with over 1 million polypropylene implants inserted each year .
	manualset3
162878	6	412103	7	NULL	NULL	0	NULL	 year	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The repair of abdominal wall defects is one of the most commonly performed general surgical procedures , with over 1 million polypropylene implants inserted each year .
	manualset3
162879	1	412104	7	NULL	NULL	0	NULL	 repair	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The repair of large full-thickness post-excisional defects of the abdominal wall .
	manualset3
162880	2	412104	7	NULL	NULL	0	NULL	large full-thickness post-excisional defects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The repair of large full-thickness post-excisional defects of the abdominal wall .
	manualset3
162881	3	412104	7	NULL	NULL	0	NULL	abdominal wall	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The repair of large full-thickness post-excisional defects of the abdominal wall .
	manualset3
162882	1	412105	7	NULL	NULL	0	NULL	 repeated isolation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The repeated isolation of the organism in pure culture from the peritoneal fluid and its isolation from postmortem subdiaphragmatic microabscesses suggest that Kluyvera can be clinically significant .
	manualset3
162883	2	412105	7	NULL	NULL	0	NULL	organism	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The repeated isolation of the organism in pure culture from the peritoneal fluid and its isolation from postmortem subdiaphragmatic microabscesses suggest that Kluyvera can be clinically significant .
	manualset3
162884	3	412105	7	NULL	NULL	0	NULL	pure culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The repeated isolation of the organism in pure culture from the peritoneal fluid and its isolation from postmortem subdiaphragmatic microabscesses suggest that Kluyvera can be clinically significant .
	manualset3
162885	4	412105	7	NULL	NULL	0	NULL	peritoneal fluid	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The repeated isolation of the organism in pure culture from the peritoneal fluid and its isolation from postmortem subdiaphragmatic microabscesses suggest that Kluyvera can be clinically significant .
	manualset3
162886	5	412105	7	NULL	NULL	0	NULL	isolation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The repeated isolation of the organism in pure culture from the peritoneal fluid and its isolation from postmortem subdiaphragmatic microabscesses suggest that Kluyvera can be clinically significant .
	manualset3
162887	6	412105	7	NULL	NULL	0	NULL	postmortem 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The repeated isolation of the organism in pure culture from the peritoneal fluid and its isolation from postmortem subdiaphragmatic microabscesses suggest that Kluyvera can be clinically significant .
	manualset3
162888	7	412105	7	NULL	NULL	0	NULL	subdiaphragmatic microabscesses	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The repeated isolation of the organism in pure culture from the peritoneal fluid and its isolation from postmortem subdiaphragmatic microabscesses suggest that Kluyvera can be clinically significant .
	manualset3
162889	8	412105	7	NULL	NULL	0	NULL	Kluyvera	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The repeated isolation of the organism in pure culture from the peritoneal fluid and its isolation from postmortem subdiaphragmatic microabscesses suggest that Kluyvera can be clinically significant .
	manualset3
162890	1	412106	7	NULL	NULL	0	NULL	 repercussions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The repercussions found , potentially associated to supernumerary teeth were : 12 ( 7.9 % ) displacement of adjacent teeth , nine ( 6 % ) delayed eruption of permanent teeth , and eight cases ( 5.3 % ) diastema formation .
	manualset3
162891	2	412106	7	NULL	NULL	0	NULL	supernumerary teeth	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The repercussions found , potentially associated to supernumerary teeth were : 12 ( 7.9 % ) displacement of adjacent teeth , nine ( 6 % ) delayed eruption of permanent teeth , and eight cases ( 5.3 % ) diastema formation .
	manualset3
162892	3	412106	7	NULL	NULL	0	NULL	12 ( 7.9 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The repercussions found , potentially associated to supernumerary teeth were : 12 ( 7.9 % ) displacement of adjacent teeth , nine ( 6 % ) delayed eruption of permanent teeth , and eight cases ( 5.3 % ) diastema formation .
	manualset3
162893	4	412106	7	NULL	NULL	0	NULL	displacement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The repercussions found , potentially associated to supernumerary teeth were : 12 ( 7.9 % ) displacement of adjacent teeth , nine ( 6 % ) delayed eruption of permanent teeth , and eight cases ( 5.3 % ) diastema formation .
	manualset3
162894	5	412106	7	NULL	NULL	0	NULL	adjacent teeth	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The repercussions found , potentially associated to supernumerary teeth were : 12 ( 7.9 % ) displacement of adjacent teeth , nine ( 6 % ) delayed eruption of permanent teeth , and eight cases ( 5.3 % ) diastema formation .
	manualset3
162895	6	412106	7	NULL	NULL	0	NULL	 nine ( 6 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The repercussions found , potentially associated to supernumerary teeth were : 12 ( 7.9 % ) displacement of adjacent teeth , nine ( 6 % ) delayed eruption of permanent teeth , and eight cases ( 5.3 % ) diastema formation .
	manualset3
162896	7	412106	7	NULL	NULL	0	NULL	delayed eruption	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The repercussions found , potentially associated to supernumerary teeth were : 12 ( 7.9 % ) displacement of adjacent teeth , nine ( 6 % ) delayed eruption of permanent teeth , and eight cases ( 5.3 % ) diastema formation .
	manualset3
162897	8	412106	7	NULL	NULL	0	NULL	permanent teeth	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The repercussions found , potentially associated to supernumerary teeth were : 12 ( 7.9 % ) displacement of adjacent teeth , nine ( 6 % ) delayed eruption of permanent teeth , and eight cases ( 5.3 % ) diastema formation .
	manualset3
162898	9	412106	7	NULL	NULL	0	NULL	eight cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The repercussions found , potentially associated to supernumerary teeth were : 12 ( 7.9 % ) displacement of adjacent teeth , nine ( 6 % ) delayed eruption of permanent teeth , and eight cases ( 5.3 % ) diastema formation .
	manualset3
162899	10	412106	7	NULL	NULL	0	NULL	5.3 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The repercussions found , potentially associated to supernumerary teeth were : 12 ( 7.9 % ) displacement of adjacent teeth , nine ( 6 % ) delayed eruption of permanent teeth , and eight cases ( 5.3 % ) diastema formation .
	manualset3
162900	11	412106	7	NULL	NULL	0	NULL	diastema formation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The repercussions found , potentially associated to supernumerary teeth were : 12 ( 7.9 % ) displacement of adjacent teeth , nine ( 6 % ) delayed eruption of permanent teeth , and eight cases ( 5.3 % ) diastema formation .
	manualset3
162905	1	412107	7	NULL	NULL	0	NULL	replacement 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The replacement of microglia significantly slowed disease progression and prolonged survival of the ALS mice compared with the ALS mice treated by stereotactic injection of PBS-liposome and BMT with BMCs expressing mSOD1 or w/tSOD1 .
	manualset3
162906	2	412107	7	NULL	NULL	0	NULL	 microglia	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The replacement of microglia significantly slowed disease progression and prolonged survival of the ALS mice compared with the ALS mice treated by stereotactic injection of PBS-liposome and BMT with BMCs expressing mSOD1 or w/tSOD1 .
	manualset3
162907	3	412107	7	NULL	NULL	0	NULL	disease progression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The replacement of microglia significantly slowed disease progression and prolonged survival of the ALS mice compared with the ALS mice treated by stereotactic injection of PBS-liposome and BMT with BMCs expressing mSOD1 or w/tSOD1 .
	manualset3
162908	4	412107	7	NULL	NULL	0	NULL	prolonged survival 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The replacement of microglia significantly slowed disease progression and prolonged survival of the ALS mice compared with the ALS mice treated by stereotactic injection of PBS-liposome and BMT with BMCs expressing mSOD1 or w/tSOD1 .
	manualset3
162909	5	412107	7	NULL	NULL	0	NULL	ALS mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The replacement of microglia significantly slowed disease progression and prolonged survival of the ALS mice compared with the ALS mice treated by stereotactic injection of PBS-liposome and BMT with BMCs expressing mSOD1 or w/tSOD1 .
	manualset3
162910	6	412107	7	NULL	NULL	0	NULL	ALS mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The replacement of microglia significantly slowed disease progression and prolonged survival of the ALS mice compared with the ALS mice treated by stereotactic injection of PBS-liposome and BMT with BMCs expressing mSOD1 or w/tSOD1 .
	manualset3
162911	7	412107	7	NULL	NULL	0	NULL	stereotactic injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The replacement of microglia significantly slowed disease progression and prolonged survival of the ALS mice compared with the ALS mice treated by stereotactic injection of PBS-liposome and BMT with BMCs expressing mSOD1 or w/tSOD1 .
	manualset3
162912	8	412107	7	NULL	NULL	0	NULL	PBS-liposome 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The replacement of microglia significantly slowed disease progression and prolonged survival of the ALS mice compared with the ALS mice treated by stereotactic injection of PBS-liposome and BMT with BMCs expressing mSOD1 or w/tSOD1 .
	manualset3
162913	9	412107	7	NULL	NULL	0	NULL	BMT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The replacement of microglia significantly slowed disease progression and prolonged survival of the ALS mice compared with the ALS mice treated by stereotactic injection of PBS-liposome and BMT with BMCs expressing mSOD1 or w/tSOD1 .
	manualset3
162914	10	412107	7	NULL	NULL	0	NULL	BMCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The replacement of microglia significantly slowed disease progression and prolonged survival of the ALS mice compared with the ALS mice treated by stereotactic injection of PBS-liposome and BMT with BMCs expressing mSOD1 or w/tSOD1 .
	manualset3
162915	11	412107	7	NULL	NULL	0	NULL	 mSOD1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The replacement of microglia significantly slowed disease progression and prolonged survival of the ALS mice compared with the ALS mice treated by stereotactic injection of PBS-liposome and BMT with BMCs expressing mSOD1 or w/tSOD1 .
	manualset3
162916	12	412107	7	NULL	NULL	0	NULL	w/tSOD1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The replacement of microglia significantly slowed disease progression and prolonged survival of the ALS mice compared with the ALS mice treated by stereotactic injection of PBS-liposome and BMT with BMCs expressing mSOD1 or w/tSOD1 .
	manualset3
162917	1	412108	7	NULL	NULL	NULL	NULL	replica	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The replica of the trichloroacetic acid-extracted cell wall ( TCA-wall ) showed two areas .
	manualset3
162918	2	412108	7	NULL	NULL	NULL	NULL	trichloroacetic acid-extracted cell wall ( TCA-wall )	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The replica of the trichloroacetic acid-extracted cell wall ( TCA-wall ) showed two areas .
	manualset3
163807	3	412108	7	NULL	NULL	NULL	NULL	two	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The replica of the trichloroacetic acid-extracted cell wall ( TCA-wall ) showed two areas .
	manualset3
163808	4	412108	7	NULL	NULL	0	NULL	areas	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The replica of the trichloroacetic acid-extracted cell wall ( TCA-wall ) showed two areas .
	manualset3
162919	1	412109	7	NULL	NULL	0	NULL	 report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The report describes the feasibility of the addition of multiple viable HLA-mismatched unrelated cord blood units , to a low cell number matched unrelated cord , to assist clinical engraftment .
	manualset3
162920	2	412109	7	NULL	NULL	NULL	NULL	 feasibility	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The report describes the feasibility of the addition of multiple viable HLA-mismatched unrelated cord blood units , to a low cell number matched unrelated cord , to assist clinical engraftment .
	manualset3
162921	3	412109	7	NULL	NULL	0	NULL	addition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The report describes the feasibility of the addition of multiple viable HLA-mismatched unrelated cord blood units , to a low cell number matched unrelated cord , to assist clinical engraftment .
	manualset3
162922	4	412109	7	NULL	NULL	0	NULL	multiple viable HLA-mismatched unrelated cord blood units	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The report describes the feasibility of the addition of multiple viable HLA-mismatched unrelated cord blood units , to a low cell number matched unrelated cord , to assist clinical engraftment .
	manualset3
162923	5	412109	7	NULL	NULL	0	NULL	low cell number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The report describes the feasibility of the addition of multiple viable HLA-mismatched unrelated cord blood units , to a low cell number matched unrelated cord , to assist clinical engraftment .
	manualset3
162924	6	412109	7	NULL	NULL	0	NULL	 unrelated cord	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The report describes the feasibility of the addition of multiple viable HLA-mismatched unrelated cord blood units , to a low cell number matched unrelated cord , to assist clinical engraftment .
	manualset3
162925	7	412109	7	NULL	NULL	0	NULL	clinical engraftment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The report describes the feasibility of the addition of multiple viable HLA-mismatched unrelated cord blood units , to a low cell number matched unrelated cord , to assist clinical engraftment .
	manualset3
162926	1	412110	7	NULL	NULL	0	NULL	reported effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The reported effect was not detected after 60 min of perfusion , and it was blunted in the presence of the protein kinase C inhibitor chelerythrine , while the calcineurin inhibitor cyclosporin A was ineffective .
	manualset3
162927	2	412110	7	NULL	NULL	0	NULL	60 min 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The reported effect was not detected after 60 min of perfusion , and it was blunted in the presence of the protein kinase C inhibitor chelerythrine , while the calcineurin inhibitor cyclosporin A was ineffective .
	manualset3
162928	3	412110	7	NULL	NULL	0	NULL	perfusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The reported effect was not detected after 60 min of perfusion , and it was blunted in the presence of the protein kinase C inhibitor chelerythrine , while the calcineurin inhibitor cyclosporin A was ineffective .
	manualset3
162929	4	412110	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The reported effect was not detected after 60 min of perfusion , and it was blunted in the presence of the protein kinase C inhibitor chelerythrine , while the calcineurin inhibitor cyclosporin A was ineffective .
	manualset3
162930	5	412110	7	NULL	NULL	0	NULL	protein kinase C inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reported effect was not detected after 60 min of perfusion , and it was blunted in the presence of the protein kinase C inhibitor chelerythrine , while the calcineurin inhibitor cyclosporin A was ineffective .
	manualset3
162931	6	412110	7	NULL	NULL	0	NULL	chelerythrine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reported effect was not detected after 60 min of perfusion , and it was blunted in the presence of the protein kinase C inhibitor chelerythrine , while the calcineurin inhibitor cyclosporin A was ineffective .
	manualset3
162932	7	412110	7	NULL	NULL	NULL	NULL	calcineurin inhibitor 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reported effect was not detected after 60 min of perfusion , and it was blunted in the presence of the protein kinase C inhibitor chelerythrine , while the calcineurin inhibitor cyclosporin A was ineffective .
	manualset3
162933	8	412110	7	NULL	NULL	0	NULL	cyclosporin A 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The reported effect was not detected after 60 min of perfusion , and it was blunted in the presence of the protein kinase C inhibitor chelerythrine , while the calcineurin inhibitor cyclosporin A was ineffective .
	manualset3
162934	1	412111	7	NULL	NULL	0	NULL	 60 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	About 60 % of the total detectable activity of hexokinase was found associated with a particulate fraction consisting essentially of mitochondria and chloroplasts and free of cytosol contamination .
	manualset3
162935	2	412111	7	NULL	NULL	0	NULL	total detectable activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	About 60 % of the total detectable activity of hexokinase was found associated with a particulate fraction consisting essentially of mitochondria and chloroplasts and free of cytosol contamination .
	manualset3
162936	3	412111	7	NULL	NULL	0	NULL	hexokinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	About 60 % of the total detectable activity of hexokinase was found associated with a particulate fraction consisting essentially of mitochondria and chloroplasts and free of cytosol contamination .
	manualset3
162937	4	412111	7	NULL	NULL	0	NULL	particulate fraction	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	About 60 % of the total detectable activity of hexokinase was found associated with a particulate fraction consisting essentially of mitochondria and chloroplasts and free of cytosol contamination .
	manualset3
162938	5	412111	7	NULL	NULL	0	NULL	mitochondria	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	About 60 % of the total detectable activity of hexokinase was found associated with a particulate fraction consisting essentially of mitochondria and chloroplasts and free of cytosol contamination .
	manualset3
162939	6	412111	7	NULL	NULL	0	NULL	chloroplasts	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	About 60 % of the total detectable activity of hexokinase was found associated with a particulate fraction consisting essentially of mitochondria and chloroplasts and free of cytosol contamination .
	manualset3
162940	7	412111	7	NULL	NULL	NULL	NULL	cytosol contamination 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	About 60 % of the total detectable activity of hexokinase was found associated with a particulate fraction consisting essentially of mitochondria and chloroplasts and free of cytosol contamination .
	manualset3
162941	1	412112	7	NULL	NULL	0	NULL	reproductive organs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The reproductive organs of SPARKI males are smaller compared with wild-type animals , and they are also subfertile .
	manualset3
162942	2	412112	7	NULL	NULL	0	NULL	SPARKI males	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The reproductive organs of SPARKI males are smaller compared with wild-type animals , and they are also subfertile .
	manualset3
162943	3	412112	7	NULL	NULL	0	NULL	 wild-type animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The reproductive organs of SPARKI males are smaller compared with wild-type animals , and they are also subfertile .
	manualset3
162945	1	412113	7	NULL	NULL	0	NULL	number of hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The required number of hours of physical education are the same for men and women .
	manualset3
162946	2	412113	7	NULL	NULL	0	NULL	physical education 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The required number of hours of physical education are the same for men and women .
	manualset3
162947	3	412113	7	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The required number of hours of physical education are the same for men and women .
	manualset3
162948	4	412113	7	NULL	NULL	0	NULL	 women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The required number of hours of physical education are the same for men and women .
	manualset3
162949	1	412114	7	NULL	NULL	0	NULL	requirement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The requirement for therapeutic drug monitoring has not been established for some of these drugs .
	manualset3
162950	2	412114	7	NULL	NULL	NULL	NULL	therapeutic drug monitoring	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The requirement for therapeutic drug monitoring has not been established for some of these drugs .
	manualset3
162951	3	412114	7	NULL	NULL	0	NULL	 drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The requirement for therapeutic drug monitoring has not been established for some of these drugs .
	manualset3
162952	1	412115	7	NULL	NULL	0	NULL	requirements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The requirements for completing BIR are significantly different from those of GC , but both processes require 5 ' to 3 ' resection of DSB ends to create single-stranded DNA that leads to formation of a Rad51 filament required to initiate HR .
	manualset3
162953	2	412115	7	NULL	NULL	NULL	NULL	BIR 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The requirements for completing BIR are significantly different from those of GC , but both processes require 5 ' to 3 ' resection of DSB ends to create single-stranded DNA that leads to formation of a Rad51 filament required to initiate HR .
	manualset3
162954	3	412115	7	NULL	NULL	0	NULL	GC	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The requirements for completing BIR are significantly different from those of GC , but both processes require 5 ' to 3 ' resection of DSB ends to create single-stranded DNA that leads to formation of a Rad51 filament required to initiate HR .
	manualset3
162955	4	412115	7	NULL	NULL	0	NULL	processes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The requirements for completing BIR are significantly different from those of GC , but both processes require 5 ' to 3 ' resection of DSB ends to create single-stranded DNA that leads to formation of a Rad51 filament required to initiate HR .
	manualset3
162956	5	412115	7	NULL	NULL	0	NULL	 5 ' to 3 ' resection	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The requirements for completing BIR are significantly different from those of GC , but both processes require 5 ' to 3 ' resection of DSB ends to create single-stranded DNA that leads to formation of a Rad51 filament required to initiate HR .
	manualset3
162957	6	412115	7	NULL	NULL	NULL	NULL	DSB	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The requirements for completing BIR are significantly different from those of GC , but both processes require 5 ' to 3 ' resection of DSB ends to create single-stranded DNA that leads to formation of a Rad51 filament required to initiate HR .
	manualset3
162958	7	412115	7	NULL	NULL	0	NULL	 single-stranded DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The requirements for completing BIR are significantly different from those of GC , but both processes require 5 ' to 3 ' resection of DSB ends to create single-stranded DNA that leads to formation of a Rad51 filament required to initiate HR .
	manualset3
162959	8	412115	7	NULL	NULL	0	NULL	formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The requirements for completing BIR are significantly different from those of GC , but both processes require 5 ' to 3 ' resection of DSB ends to create single-stranded DNA that leads to formation of a Rad51 filament required to initiate HR .
	manualset3
162960	9	412115	7	NULL	NULL	0	NULL	Rad51 filament	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The requirements for completing BIR are significantly different from those of GC , but both processes require 5 ' to 3 ' resection of DSB ends to create single-stranded DNA that leads to formation of a Rad51 filament required to initiate HR .
	manualset3
162961	10	412115	7	NULL	NULL	0	NULL	HR 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The requirements for completing BIR are significantly different from those of GC , but both processes require 5 ' to 3 ' resection of DSB ends to create single-stranded DNA that leads to formation of a Rad51 filament required to initiate HR .
	manualset3
162962	1	412116	7	NULL	NULL	NULL	NULL	residual risk 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The residual risk of CF was 11 % when only one CF mutation was detected by the first screening step , thereby justifying in-depth screening .
	manualset3
162963	2	412116	7	NULL	NULL	0	NULL	CF	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The residual risk of CF was 11 % when only one CF mutation was detected by the first screening step , thereby justifying in-depth screening .
	manualset3
162964	3	412116	7	NULL	NULL	0	NULL	11 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The residual risk of CF was 11 % when only one CF mutation was detected by the first screening step , thereby justifying in-depth screening .
	manualset3
162965	4	412116	7	NULL	NULL	0	NULL	 CF mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The residual risk of CF was 11 % when only one CF mutation was detected by the first screening step , thereby justifying in-depth screening .
	manualset3
162966	5	412116	7	NULL	NULL	0	NULL	first screening step	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The residual risk of CF was 11 % when only one CF mutation was detected by the first screening step , thereby justifying in-depth screening .
	manualset3
162967	6	412116	7	NULL	NULL	NULL	NULL	in-depth screening	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The residual risk of CF was 11 % when only one CF mutation was detected by the first screening step , thereby justifying in-depth screening .
	manualset3
162968	1	412117	7	NULL	NULL	0	NULL	 resolution 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resolution of the sensor has been calibrated using an interferometer and was shown to be as high as 0.3 A per system count .
	manualset3
162969	2	412117	7	NULL	NULL	0	NULL	sensor	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The resolution of the sensor has been calibrated using an interferometer and was shown to be as high as 0.3 A per system count .
	manualset3
162970	3	412117	7	NULL	NULL	0	NULL	interferometer	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The resolution of the sensor has been calibrated using an interferometer and was shown to be as high as 0.3 A per system count .
	manualset3
162971	4	412117	7	NULL	NULL	0	NULL	0.3 A per system count	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The resolution of the sensor has been calibrated using an interferometer and was shown to be as high as 0.3 A per system count .
	manualset3
162972	1	412118	7	NULL	NULL	0	NULL	resonator device	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The resonator device is based around a ring of NbN containing a microbridge bottleneck , whose switching between normal and super conducting states can be modeled as discontinuous , and whose fast temperature versus slow current fluctuations are modeled by a slow-fast timescale separation in the dynamics .
	manualset3
162973	2	412118	7	NULL	NULL	0	NULL	ring of NbN	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The resonator device is based around a ring of NbN containing a microbridge bottleneck , whose switching between normal and super conducting states can be modeled as discontinuous , and whose fast temperature versus slow current fluctuations are modeled by a slow-fast timescale separation in the dynamics .
	manualset3
162974	3	412118	7	NULL	NULL	NULL	NULL	microbridge bottleneck	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The resonator device is based around a ring of NbN containing a microbridge bottleneck , whose switching between normal and super conducting states can be modeled as discontinuous , and whose fast temperature versus slow current fluctuations are modeled by a slow-fast timescale separation in the dynamics .
	manualset3
162975	4	412118	7	NULL	NULL	0	NULL	normal conducting state	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The resonator device is based around a ring of NbN containing a microbridge bottleneck , whose switching between normal and super conducting states can be modeled as discontinuous , and whose fast temperature versus slow current fluctuations are modeled by a slow-fast timescale separation in the dynamics .
	manualset3
162976	5	412118	7	NULL	NULL	0	NULL	super conducting states	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The resonator device is based around a ring of NbN containing a microbridge bottleneck , whose switching between normal and super conducting states can be modeled as discontinuous , and whose fast temperature versus slow current fluctuations are modeled by a slow-fast timescale separation in the dynamics .
	manualset3
162977	6	412118	7	NULL	NULL	0	NULL	fast temperature	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resonator device is based around a ring of NbN containing a microbridge bottleneck , whose switching between normal and super conducting states can be modeled as discontinuous , and whose fast temperature versus slow current fluctuations are modeled by a slow-fast timescale separation in the dynamics .
	manualset3
162978	7	412118	7	NULL	NULL	0	NULL	slow current fluctuations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resonator device is based around a ring of NbN containing a microbridge bottleneck , whose switching between normal and super conducting states can be modeled as discontinuous , and whose fast temperature versus slow current fluctuations are modeled by a slow-fast timescale separation in the dynamics .
	manualset3
162979	8	412118	7	NULL	NULL	0	NULL	slow-fast timescale separation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The resonator device is based around a ring of NbN containing a microbridge bottleneck , whose switching between normal and super conducting states can be modeled as discontinuous , and whose fast temperature versus slow current fluctuations are modeled by a slow-fast timescale separation in the dynamics .
	manualset3
162980	9	412118	7	NULL	NULL	0	NULL	dynamics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The resonator device is based around a ring of NbN containing a microbridge bottleneck , whose switching between normal and super conducting states can be modeled as discontinuous , and whose fast temperature versus slow current fluctuations are modeled by a slow-fast timescale separation in the dynamics .
	manualset3
162981	1	412119	7	NULL	NULL	0	NULL	 resources	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The resources have been made available free on the Web by healthcare professionals and government agencies from around the world .
	manualset3
162983	3	412119	7	NULL	NULL	0	NULL	 Web	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The resources have been made available free on the Web by healthcare professionals and government agencies from around the world .
	manualset3
162984	4	412119	7	NULL	NULL	0	NULL	healthcare professionals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The resources have been made available free on the Web by healthcare professionals and government agencies from around the world .
	manualset3
162985	5	412119	7	NULL	NULL	0	NULL	government agencies	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The resources have been made available free on the Web by healthcare professionals and government agencies from around the world .
	manualset3
162986	6	412119	7	NULL	NULL	0	NULL	world 	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The resources have been made available free on the Web by healthcare professionals and government agencies from around the world .
	manualset3
162987	1	412120	7	NULL	NULL	0	NULL	respective indices	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The respective indices for UTI were calculated as 95.0 , 92.9 , 89.7 , and 96.6 % .
	manualset3
162988	2	412120	7	NULL	NULL	NULL	NULL	UTI	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The respective indices for UTI were calculated as 95.0 , 92.9 , 89.7 , and 96.6 % .
	manualset3
162989	3	412120	7	NULL	NULL	0	NULL	95.0 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The respective indices for UTI were calculated as 95.0 , 92.9 , 89.7 , and 96.6 % .
	manualset3
162990	4	412120	7	NULL	NULL	0	NULL	92.9%	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The respective indices for UTI were calculated as 95.0 , 92.9 , 89.7 , and 96.6 % .
	manualset3
162991	5	412120	7	NULL	NULL	0	NULL	 89.7%	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The respective indices for UTI were calculated as 95.0 , 92.9 , 89.7 , and 96.6 % .
	manualset3
162992	6	412120	7	NULL	NULL	0	NULL	 96.6 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The respective indices for UTI were calculated as 95.0 , 92.9 , 89.7 , and 96.6 % .
	manualset3
162993	1	412121	7	NULL	NULL	0	NULL	respiration 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiration of freshly cut leaves is insensitive to KCN up to 8 millimolar , but sensitive to benzhydroxamate ( BAM ) , 1 to 2 millimolar BAM causing 25 % promotion and higher concentrations inhibiting .
	manualset3
162994	2	412121	7	NULL	NULL	0	NULL	freshly cut leaves	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiration of freshly cut leaves is insensitive to KCN up to 8 millimolar , but sensitive to benzhydroxamate ( BAM ) , 1 to 2 millimolar BAM causing 25 % promotion and higher concentrations inhibiting .
	manualset3
162995	3	412121	7	NULL	NULL	0	NULL	KCN	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiration of freshly cut leaves is insensitive to KCN up to 8 millimolar , but sensitive to benzhydroxamate ( BAM ) , 1 to 2 millimolar BAM causing 25 % promotion and higher concentrations inhibiting .
	manualset3
162996	4	412121	7	NULL	NULL	0	NULL	 8 millimolar	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiration of freshly cut leaves is insensitive to KCN up to 8 millimolar , but sensitive to benzhydroxamate ( BAM ) , 1 to 2 millimolar BAM causing 25 % promotion and higher concentrations inhibiting .
	manualset3
162997	5	412121	7	NULL	NULL	0	NULL	benzhydroxamate ( BAM )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiration of freshly cut leaves is insensitive to KCN up to 8 millimolar , but sensitive to benzhydroxamate ( BAM ) , 1 to 2 millimolar BAM causing 25 % promotion and higher concentrations inhibiting .
	manualset3
162998	6	412121	7	NULL	NULL	0	NULL	1 to 2 millimolar	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiration of freshly cut leaves is insensitive to KCN up to 8 millimolar , but sensitive to benzhydroxamate ( BAM ) , 1 to 2 millimolar BAM causing 25 % promotion and higher concentrations inhibiting .
	manualset3
162999	7	412121	7	NULL	NULL	0	NULL	BAM	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiration of freshly cut leaves is insensitive to KCN up to 8 millimolar , but sensitive to benzhydroxamate ( BAM ) , 1 to 2 millimolar BAM causing 25 % promotion and higher concentrations inhibiting .
	manualset3
163000	8	412121	7	NULL	NULL	0	NULL	25 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiration of freshly cut leaves is insensitive to KCN up to 8 millimolar , but sensitive to benzhydroxamate ( BAM ) , 1 to 2 millimolar BAM causing 25 % promotion and higher concentrations inhibiting .
	manualset3
163001	9	412121	7	NULL	NULL	0	NULL	promotion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiration of freshly cut leaves is insensitive to KCN up to 8 millimolar , but sensitive to benzhydroxamate ( BAM ) , 1 to 2 millimolar BAM causing 25 % promotion and higher concentrations inhibiting .
	manualset3
163002	10	412121	7	NULL	NULL	0	NULL	concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiration of freshly cut leaves is insensitive to KCN up to 8 millimolar , but sensitive to benzhydroxamate ( BAM ) , 1 to 2 millimolar BAM causing 25 % promotion and higher concentrations inhibiting .
	manualset3
163003	1	412122	7	NULL	NULL	0	NULL	 respiratory activities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiratory activities and ultrastructure of isolated mitochondria and the cellular bioenergetic state in fetal rat brain were examined at the end of 30 minutes of in utero ischemia and after 1 , 2 , 3 and 4 hours of recirculation .
	manualset3
163004	2	412122	7	NULL	NULL	0	NULL	 ultrastructure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiratory activities and ultrastructure of isolated mitochondria and the cellular bioenergetic state in fetal rat brain were examined at the end of 30 minutes of in utero ischemia and after 1 , 2 , 3 and 4 hours of recirculation .
	manualset3
163005	3	412122	7	NULL	NULL	0	NULL	 isolated mitochondria	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiratory activities and ultrastructure of isolated mitochondria and the cellular bioenergetic state in fetal rat brain were examined at the end of 30 minutes of in utero ischemia and after 1 , 2 , 3 and 4 hours of recirculation .
	manualset3
163006	4	412122	7	NULL	NULL	0	NULL	cellular bioenergetic state	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiratory activities and ultrastructure of isolated mitochondria and the cellular bioenergetic state in fetal rat brain were examined at the end of 30 minutes of in utero ischemia and after 1 , 2 , 3 and 4 hours of recirculation .
	manualset3
163007	5	412122	7	NULL	NULL	0	NULL	fetal rat brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiratory activities and ultrastructure of isolated mitochondria and the cellular bioenergetic state in fetal rat brain were examined at the end of 30 minutes of in utero ischemia and after 1 , 2 , 3 and 4 hours of recirculation .
	manualset3
163008	6	412122	7	NULL	NULL	0	NULL	30 minutes	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiratory activities and ultrastructure of isolated mitochondria and the cellular bioenergetic state in fetal rat brain were examined at the end of 30 minutes of in utero ischemia and after 1 , 2 , 3 and 4 hours of recirculation .
	manualset3
163009	7	412122	7	NULL	NULL	0	NULL	in utero ischemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiratory activities and ultrastructure of isolated mitochondria and the cellular bioenergetic state in fetal rat brain were examined at the end of 30 minutes of in utero ischemia and after 1 , 2 , 3 and 4 hours of recirculation .
	manualset3
163010	8	412122	7	NULL	NULL	0	NULL	1 hour	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiratory activities and ultrastructure of isolated mitochondria and the cellular bioenergetic state in fetal rat brain were examined at the end of 30 minutes of in utero ischemia and after 1 , 2 , 3 and 4 hours of recirculation .
	manualset3
163011	9	412122	7	NULL	NULL	NULL	NULL	2 hours	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The respiratory activities and ultrastructure of isolated mitochondria and the cellular bioenergetic state in fetal rat brain were examined at the end of 30 minutes of in utero ischemia and after 1 , 2 , 3 and 4 hours of recirculation .
	manualset3
163012	10	412122	7	NULL	NULL	0	NULL	3 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiratory activities and ultrastructure of isolated mitochondria and the cellular bioenergetic state in fetal rat brain were examined at the end of 30 minutes of in utero ischemia and after 1 , 2 , 3 and 4 hours of recirculation .
	manualset3
163013	11	412122	7	NULL	NULL	0	NULL	4 hours 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiratory activities and ultrastructure of isolated mitochondria and the cellular bioenergetic state in fetal rat brain were examined at the end of 30 minutes of in utero ischemia and after 1 , 2 , 3 and 4 hours of recirculation .
	manualset3
163014	12	412122	7	NULL	NULL	0	NULL	recirculation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiratory activities and ultrastructure of isolated mitochondria and the cellular bioenergetic state in fetal rat brain were examined at the end of 30 minutes of in utero ischemia and after 1 , 2 , 3 and 4 hours of recirculation .
	manualset3
163015	1	412123	7	NULL	NULL	0	NULL	 respiratory control ratio ( RCR )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiratory control ratio ( RCR ) of mitochondria from vehicle-treated animals was significantly ( p & lt ; 0.01 ) lower at 3 or 12 h post-TBI , relative to shams .
	manualset3
163016	2	412123	7	NULL	NULL	0	NULL	mitochondria	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiratory control ratio ( RCR ) of mitochondria from vehicle-treated animals was significantly ( p & lt ; 0.01 ) lower at 3 or 12 h post-TBI , relative to shams .
	manualset3
163017	3	412123	7	NULL	NULL	0	NULL	vehicle-treated animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiratory control ratio ( RCR ) of mitochondria from vehicle-treated animals was significantly ( p & lt ; 0.01 ) lower at 3 or 12 h post-TBI , relative to shams .
	manualset3
163018	4	412123	7	NULL	NULL	0	NULL	p & lt ; 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiratory control ratio ( RCR ) of mitochondria from vehicle-treated animals was significantly ( p & lt ; 0.01 ) lower at 3 or 12 h post-TBI , relative to shams .
	manualset3
163019	5	412123	7	NULL	NULL	0	NULL	3 h post-TBI	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiratory control ratio ( RCR ) of mitochondria from vehicle-treated animals was significantly ( p & lt ; 0.01 ) lower at 3 or 12 h post-TBI , relative to shams .
	manualset3
163020	6	412123	7	NULL	NULL	0	NULL	12 h post-TBI	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiratory control ratio ( RCR ) of mitochondria from vehicle-treated animals was significantly ( p & lt ; 0.01 ) lower at 3 or 12 h post-TBI , relative to shams .
	manualset3
163021	7	412123	7	NULL	NULL	0	NULL	shams	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiratory control ratio ( RCR ) of mitochondria from vehicle-treated animals was significantly ( p & lt ; 0.01 ) lower at 3 or 12 h post-TBI , relative to shams .
	manualset3
163022	1	412124	7	NULL	NULL	NULL	NULL	response	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The response consisted of a marked increase in conductance associated with a potential change .
	manualset3
163023	2	412124	7	NULL	NULL	NULL	NULL	marked increase	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The response consisted of a marked increase in conductance associated with a potential change .
	manualset3
163024	3	412124	7	NULL	NULL	0	NULL	conductance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The response consisted of a marked increase in conductance associated with a potential change .
	manualset3
163025	4	412124	7	NULL	NULL	0	NULL	potential change	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The response consisted of a marked increase in conductance associated with a potential change .
	manualset3
163026	1	412125	7	NULL	NULL	0	NULL	response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The response induced by 2-arachidonoylglycerol in either NG108-15 cells or N18TG2 cells was abolished by pretreatment of the cells with a cannabinoid CB1 receptor specific antagonist , SR141716A , suggesting that 2-arachidonoylglycerol interacts with the CB1 receptor to induce the response .
	manualset3
163027	2	412125	7	NULL	NULL	0	NULL	 2-arachidonoylglycerol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The response induced by 2-arachidonoylglycerol in either NG108-15 cells or N18TG2 cells was abolished by pretreatment of the cells with a cannabinoid CB1 receptor specific antagonist , SR141716A , suggesting that 2-arachidonoylglycerol interacts with the CB1 receptor to induce the response .
	manualset3
163028	3	412125	7	NULL	NULL	0	NULL	NG108-15 cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The response induced by 2-arachidonoylglycerol in either NG108-15 cells or N18TG2 cells was abolished by pretreatment of the cells with a cannabinoid CB1 receptor specific antagonist , SR141716A , suggesting that 2-arachidonoylglycerol interacts with the CB1 receptor to induce the response .
	manualset3
163029	4	412125	7	NULL	NULL	0	NULL	N18TG2 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The response induced by 2-arachidonoylglycerol in either NG108-15 cells or N18TG2 cells was abolished by pretreatment of the cells with a cannabinoid CB1 receptor specific antagonist , SR141716A , suggesting that 2-arachidonoylglycerol interacts with the CB1 receptor to induce the response .
	manualset3
163030	5	412125	7	NULL	NULL	0	NULL	pretreatment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The response induced by 2-arachidonoylglycerol in either NG108-15 cells or N18TG2 cells was abolished by pretreatment of the cells with a cannabinoid CB1 receptor specific antagonist , SR141716A , suggesting that 2-arachidonoylglycerol interacts with the CB1 receptor to induce the response .
	manualset3
163031	6	412125	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The response induced by 2-arachidonoylglycerol in either NG108-15 cells or N18TG2 cells was abolished by pretreatment of the cells with a cannabinoid CB1 receptor specific antagonist , SR141716A , suggesting that 2-arachidonoylglycerol interacts with the CB1 receptor to induce the response .
	manualset3
163032	7	412125	7	NULL	NULL	0	NULL	cannabinoid CB1 receptor specific antagonist 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The response induced by 2-arachidonoylglycerol in either NG108-15 cells or N18TG2 cells was abolished by pretreatment of the cells with a cannabinoid CB1 receptor specific antagonist , SR141716A , suggesting that 2-arachidonoylglycerol interacts with the CB1 receptor to induce the response .
	manualset3
163033	8	412125	7	NULL	NULL	0	NULL	SR141716A	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The response induced by 2-arachidonoylglycerol in either NG108-15 cells or N18TG2 cells was abolished by pretreatment of the cells with a cannabinoid CB1 receptor specific antagonist , SR141716A , suggesting that 2-arachidonoylglycerol interacts with the CB1 receptor to induce the response .
	manualset3
163034	9	412125	7	NULL	NULL	0	NULL	 2-arachidonoylglycerol 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The response induced by 2-arachidonoylglycerol in either NG108-15 cells or N18TG2 cells was abolished by pretreatment of the cells with a cannabinoid CB1 receptor specific antagonist , SR141716A , suggesting that 2-arachidonoylglycerol interacts with the CB1 receptor to induce the response .
	manualset3
163035	10	412125	7	NULL	NULL	0	NULL	CB1 receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The response induced by 2-arachidonoylglycerol in either NG108-15 cells or N18TG2 cells was abolished by pretreatment of the cells with a cannabinoid CB1 receptor specific antagonist , SR141716A , suggesting that 2-arachidonoylglycerol interacts with the CB1 receptor to induce the response .
	manualset3
163036	11	412125	7	NULL	NULL	0	NULL	 response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The response induced by 2-arachidonoylglycerol in either NG108-15 cells or N18TG2 cells was abolished by pretreatment of the cells with a cannabinoid CB1 receptor specific antagonist , SR141716A , suggesting that 2-arachidonoylglycerol interacts with the CB1 receptor to induce the response .
	manualset3
163037	1	412126	7	NULL	NULL	0	NULL	 response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The response of ameloblasts to long-term ( 6 weeks ) exposure to 100 ppm fluoride was examined in continuously erupting mandibular incisors of female Sprague-Dawley rats as compared to control rats receiving a similar diet ( Teklad L-356 ) but no sodium fluoride in their drinking water .
	manualset3
163038	2	412126	7	NULL	NULL	0	NULL	ameloblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The response of ameloblasts to long-term ( 6 weeks ) exposure to 100 ppm fluoride was examined in continuously erupting mandibular incisors of female Sprague-Dawley rats as compared to control rats receiving a similar diet ( Teklad L-356 ) but no sodium fluoride in their drinking water .
	manualset3
163039	3	412126	7	NULL	NULL	0	NULL	long-term ( 6 weeks ) exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The response of ameloblasts to long-term ( 6 weeks ) exposure to 100 ppm fluoride was examined in continuously erupting mandibular incisors of female Sprague-Dawley rats as compared to control rats receiving a similar diet ( Teklad L-356 ) but no sodium fluoride in their drinking water .
	manualset3
163040	4	412126	7	NULL	NULL	0	NULL	100 ppm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The response of ameloblasts to long-term ( 6 weeks ) exposure to 100 ppm fluoride was examined in continuously erupting mandibular incisors of female Sprague-Dawley rats as compared to control rats receiving a similar diet ( Teklad L-356 ) but no sodium fluoride in their drinking water .
	manualset3
163041	5	412126	7	NULL	NULL	0	NULL	fluoride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The response of ameloblasts to long-term ( 6 weeks ) exposure to 100 ppm fluoride was examined in continuously erupting mandibular incisors of female Sprague-Dawley rats as compared to control rats receiving a similar diet ( Teklad L-356 ) but no sodium fluoride in their drinking water .
	manualset3
163042	6	412126	7	NULL	NULL	0	NULL	mandibular incisors	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The response of ameloblasts to long-term ( 6 weeks ) exposure to 100 ppm fluoride was examined in continuously erupting mandibular incisors of female Sprague-Dawley rats as compared to control rats receiving a similar diet ( Teklad L-356 ) but no sodium fluoride in their drinking water .
	manualset3
163043	7	412126	7	NULL	NULL	0	NULL	female Sprague-Dawley rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The response of ameloblasts to long-term ( 6 weeks ) exposure to 100 ppm fluoride was examined in continuously erupting mandibular incisors of female Sprague-Dawley rats as compared to control rats receiving a similar diet ( Teklad L-356 ) but no sodium fluoride in their drinking water .
	manualset3
163044	8	412126	7	NULL	NULL	0	NULL	control rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The response of ameloblasts to long-term ( 6 weeks ) exposure to 100 ppm fluoride was examined in continuously erupting mandibular incisors of female Sprague-Dawley rats as compared to control rats receiving a similar diet ( Teklad L-356 ) but no sodium fluoride in their drinking water .
	manualset3
163045	9	412126	7	NULL	NULL	0	NULL	similar diet 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The response of ameloblasts to long-term ( 6 weeks ) exposure to 100 ppm fluoride was examined in continuously erupting mandibular incisors of female Sprague-Dawley rats as compared to control rats receiving a similar diet ( Teklad L-356 ) but no sodium fluoride in their drinking water .
	manualset3
163046	10	412126	7	NULL	NULL	0	NULL	Teklad L-356	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The response of ameloblasts to long-term ( 6 weeks ) exposure to 100 ppm fluoride was examined in continuously erupting mandibular incisors of female Sprague-Dawley rats as compared to control rats receiving a similar diet ( Teklad L-356 ) but no sodium fluoride in their drinking water .
	manualset3
163047	11	412126	7	NULL	NULL	0	NULL	sodium fluoride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The response of ameloblasts to long-term ( 6 weeks ) exposure to 100 ppm fluoride was examined in continuously erupting mandibular incisors of female Sprague-Dawley rats as compared to control rats receiving a similar diet ( Teklad L-356 ) but no sodium fluoride in their drinking water .
	manualset3
163048	12	412126	7	NULL	NULL	0	NULL	drinking water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The response of ameloblasts to long-term ( 6 weeks ) exposure to 100 ppm fluoride was examined in continuously erupting mandibular incisors of female Sprague-Dawley rats as compared to control rats receiving a similar diet ( Teklad L-356 ) but no sodium fluoride in their drinking water .
	manualset3
163049	1	412127	7	NULL	NULL	0	NULL	1-3 x 10 ( 6 ) mature dendritic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	About 1-3 x 10 ( 6 ) mature dendritic cells are generated from 40 ml of blood vs. & lt ; 0.1 x 10 ( 6 ) from noncytokine treated blood .
	manualset3
163050	2	412127	7	NULL	NULL	0	NULL	40 ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	About 1-3 x 10 ( 6 ) mature dendritic cells are generated from 40 ml of blood vs. & lt ; 0.1 x 10 ( 6 ) from noncytokine treated blood .
	manualset3
163051	3	412127	7	NULL	NULL	0	NULL	blood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	About 1-3 x 10 ( 6 ) mature dendritic cells are generated from 40 ml of blood vs. & lt ; 0.1 x 10 ( 6 ) from noncytokine treated blood .
	manualset3
163052	4	412127	7	NULL	NULL	0	NULL	lt ; 0.1 x 10 ( 6 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	About 1-3 x 10 ( 6 ) mature dendritic cells are generated from 40 ml of blood vs. & lt ; 0.1 x 10 ( 6 ) from noncytokine treated blood .
	manualset3
163054	5	412127	7	NULL	NULL	NULL	NULL	 noncytokine treated blood	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	About 1-3 x 10 ( 6 ) mature dendritic cells are generated from 40 ml of blood vs. & lt ; 0.1 x 10 ( 6 ) from noncytokine treated blood .
	manualset3
163055	1	412128	7	NULL	NULL	0	NULL	response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The response to exercise stress is characterized by an increase in circulating catecholamines and rapid synthesis of the inducible member of the 70 kDa family of heat shock proteins ( Hsp70 ) .
	manualset3
163056	2	412128	7	NULL	NULL	0	NULL	 exercise stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The response to exercise stress is characterized by an increase in circulating catecholamines and rapid synthesis of the inducible member of the 70 kDa family of heat shock proteins ( Hsp70 ) .
	manualset3
163057	3	412128	7	NULL	NULL	0	NULL	circulating catecholamines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The response to exercise stress is characterized by an increase in circulating catecholamines and rapid synthesis of the inducible member of the 70 kDa family of heat shock proteins ( Hsp70 ) .
	manualset3
163058	4	412128	7	NULL	NULL	0	NULL	rapid synthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The response to exercise stress is characterized by an increase in circulating catecholamines and rapid synthesis of the inducible member of the 70 kDa family of heat shock proteins ( Hsp70 ) .
	manualset3
163059	5	412128	7	NULL	NULL	0	NULL	inducible member 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The response to exercise stress is characterized by an increase in circulating catecholamines and rapid synthesis of the inducible member of the 70 kDa family of heat shock proteins ( Hsp70 ) .
	manualset3
163060	6	412128	7	NULL	NULL	NULL	NULL	70 kDa family of heat shock proteins ( Hsp70 ) 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The response to exercise stress is characterized by an increase in circulating catecholamines and rapid synthesis of the inducible member of the 70 kDa family of heat shock proteins ( Hsp70 ) .
	manualset3
163061	1	412129	7	NULL	NULL	0	NULL	 response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The response to exogenous parathyroid hormone ( PTH ) with urinary excretion of phosphate and cyclic adenosine monophosphate ( cAMP ) was tested by the use of synthetic human parathyroid hormone ( 1-34 ) ( hPTH - ( 1-34 ) ) on 59 patients with hypocalcemia and normal or high serum inorganic phosphorus and normal renal function without a history of parathyroidectomy for differentiation between idiopathic hypoparathyroidism ( IHP ) , pseudohypoparathyroidism ( PHP ) and related diseases along with 18 normal subjects .
	manualset3
163062	2	412129	7	NULL	NULL	0	NULL	exogenous parathyroid hormone ( PTH )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The response to exogenous parathyroid hormone ( PTH ) with urinary excretion of phosphate and cyclic adenosine monophosphate ( cAMP ) was tested by the use of synthetic human parathyroid hormone ( 1-34 ) ( hPTH - ( 1-34 ) ) on 59 patients with hypocalcemia and normal or high serum inorganic phosphorus and normal renal function without a history of parathyroidectomy for differentiation between idiopathic hypoparathyroidism ( IHP ) , pseudohypoparathyroidism ( PHP ) and related diseases along with 18 normal subjects .
	manualset3
163063	3	412129	7	NULL	NULL	0	NULL	urinary excretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The response to exogenous parathyroid hormone ( PTH ) with urinary excretion of phosphate and cyclic adenosine monophosphate ( cAMP ) was tested by the use of synthetic human parathyroid hormone ( 1-34 ) ( hPTH - ( 1-34 ) ) on 59 patients with hypocalcemia and normal or high serum inorganic phosphorus and normal renal function without a history of parathyroidectomy for differentiation between idiopathic hypoparathyroidism ( IHP ) , pseudohypoparathyroidism ( PHP ) and related diseases along with 18 normal subjects .
	manualset3
163064	4	412129	7	NULL	NULL	0	NULL	phosphate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The response to exogenous parathyroid hormone ( PTH ) with urinary excretion of phosphate and cyclic adenosine monophosphate ( cAMP ) was tested by the use of synthetic human parathyroid hormone ( 1-34 ) ( hPTH - ( 1-34 ) ) on 59 patients with hypocalcemia and normal or high serum inorganic phosphorus and normal renal function without a history of parathyroidectomy for differentiation between idiopathic hypoparathyroidism ( IHP ) , pseudohypoparathyroidism ( PHP ) and related diseases along with 18 normal subjects .
	manualset3
163065	5	412129	7	NULL	NULL	0	NULL	cyclic adenosine monophosphate ( cAMP )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The response to exogenous parathyroid hormone ( PTH ) with urinary excretion of phosphate and cyclic adenosine monophosphate ( cAMP ) was tested by the use of synthetic human parathyroid hormone ( 1-34 ) ( hPTH - ( 1-34 ) ) on 59 patients with hypocalcemia and normal or high serum inorganic phosphorus and normal renal function without a history of parathyroidectomy for differentiation between idiopathic hypoparathyroidism ( IHP ) , pseudohypoparathyroidism ( PHP ) and related diseases along with 18 normal subjects .
	manualset3
163066	6	412129	7	NULL	NULL	NULL	NULL	use	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The response to exogenous parathyroid hormone ( PTH ) with urinary excretion of phosphate and cyclic adenosine monophosphate ( cAMP ) was tested by the use of synthetic human parathyroid hormone ( 1-34 ) ( hPTH - ( 1-34 ) ) on 59 patients with hypocalcemia and normal or high serum inorganic phosphorus and normal renal function without a history of parathyroidectomy for differentiation between idiopathic hypoparathyroidism ( IHP ) , pseudohypoparathyroidism ( PHP ) and related diseases along with 18 normal subjects .
	manualset3
163067	7	412129	7	NULL	NULL	0	NULL	synthetic human parathyroid hormone ( 1-34 ) ( hPTH - ( 1-34 ) )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The response to exogenous parathyroid hormone ( PTH ) with urinary excretion of phosphate and cyclic adenosine monophosphate ( cAMP ) was tested by the use of synthetic human parathyroid hormone ( 1-34 ) ( hPTH - ( 1-34 ) ) on 59 patients with hypocalcemia and normal or high serum inorganic phosphorus and normal renal function without a history of parathyroidectomy for differentiation between idiopathic hypoparathyroidism ( IHP ) , pseudohypoparathyroidism ( PHP ) and related diseases along with 18 normal subjects .
	manualset3
163068	8	412129	7	NULL	NULL	0	NULL	59 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The response to exogenous parathyroid hormone ( PTH ) with urinary excretion of phosphate and cyclic adenosine monophosphate ( cAMP ) was tested by the use of synthetic human parathyroid hormone ( 1-34 ) ( hPTH - ( 1-34 ) ) on 59 patients with hypocalcemia and normal or high serum inorganic phosphorus and normal renal function without a history of parathyroidectomy for differentiation between idiopathic hypoparathyroidism ( IHP ) , pseudohypoparathyroidism ( PHP ) and related diseases along with 18 normal subjects .
	manualset3
163069	9	412129	7	NULL	NULL	0	NULL	hypocalcemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The response to exogenous parathyroid hormone ( PTH ) with urinary excretion of phosphate and cyclic adenosine monophosphate ( cAMP ) was tested by the use of synthetic human parathyroid hormone ( 1-34 ) ( hPTH - ( 1-34 ) ) on 59 patients with hypocalcemia and normal or high serum inorganic phosphorus and normal renal function without a history of parathyroidectomy for differentiation between idiopathic hypoparathyroidism ( IHP ) , pseudohypoparathyroidism ( PHP ) and related diseases along with 18 normal subjects .
	manualset3
163070	10	412129	7	NULL	NULL	0	NULL	 normal serum inorganic phosphorus	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The response to exogenous parathyroid hormone ( PTH ) with urinary excretion of phosphate and cyclic adenosine monophosphate ( cAMP ) was tested by the use of synthetic human parathyroid hormone ( 1-34 ) ( hPTH - ( 1-34 ) ) on 59 patients with hypocalcemia and normal or high serum inorganic phosphorus and normal renal function without a history of parathyroidectomy for differentiation between idiopathic hypoparathyroidism ( IHP ) , pseudohypoparathyroidism ( PHP ) and related diseases along with 18 normal subjects .
	manualset3
163071	11	412129	7	NULL	NULL	0	NULL	high serum inorganic phosphorus	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The response to exogenous parathyroid hormone ( PTH ) with urinary excretion of phosphate and cyclic adenosine monophosphate ( cAMP ) was tested by the use of synthetic human parathyroid hormone ( 1-34 ) ( hPTH - ( 1-34 ) ) on 59 patients with hypocalcemia and normal or high serum inorganic phosphorus and normal renal function without a history of parathyroidectomy for differentiation between idiopathic hypoparathyroidism ( IHP ) , pseudohypoparathyroidism ( PHP ) and related diseases along with 18 normal subjects .
	manualset3
163072	12	412129	7	NULL	NULL	0	NULL	normal renal function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The response to exogenous parathyroid hormone ( PTH ) with urinary excretion of phosphate and cyclic adenosine monophosphate ( cAMP ) was tested by the use of synthetic human parathyroid hormone ( 1-34 ) ( hPTH - ( 1-34 ) ) on 59 patients with hypocalcemia and normal or high serum inorganic phosphorus and normal renal function without a history of parathyroidectomy for differentiation between idiopathic hypoparathyroidism ( IHP ) , pseudohypoparathyroidism ( PHP ) and related diseases along with 18 normal subjects .
	manualset3
163073	13	412129	7	NULL	NULL	0	NULL	history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The response to exogenous parathyroid hormone ( PTH ) with urinary excretion of phosphate and cyclic adenosine monophosphate ( cAMP ) was tested by the use of synthetic human parathyroid hormone ( 1-34 ) ( hPTH - ( 1-34 ) ) on 59 patients with hypocalcemia and normal or high serum inorganic phosphorus and normal renal function without a history of parathyroidectomy for differentiation between idiopathic hypoparathyroidism ( IHP ) , pseudohypoparathyroidism ( PHP ) and related diseases along with 18 normal subjects .
	manualset3
163074	14	412129	7	NULL	NULL	0	NULL	parathyroidectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The response to exogenous parathyroid hormone ( PTH ) with urinary excretion of phosphate and cyclic adenosine monophosphate ( cAMP ) was tested by the use of synthetic human parathyroid hormone ( 1-34 ) ( hPTH - ( 1-34 ) ) on 59 patients with hypocalcemia and normal or high serum inorganic phosphorus and normal renal function without a history of parathyroidectomy for differentiation between idiopathic hypoparathyroidism ( IHP ) , pseudohypoparathyroidism ( PHP ) and related diseases along with 18 normal subjects .
	manualset3
163075	15	412129	7	NULL	NULL	0	NULL	idiopathic hypoparathyroidism ( IHP )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The response to exogenous parathyroid hormone ( PTH ) with urinary excretion of phosphate and cyclic adenosine monophosphate ( cAMP ) was tested by the use of synthetic human parathyroid hormone ( 1-34 ) ( hPTH - ( 1-34 ) ) on 59 patients with hypocalcemia and normal or high serum inorganic phosphorus and normal renal function without a history of parathyroidectomy for differentiation between idiopathic hypoparathyroidism ( IHP ) , pseudohypoparathyroidism ( PHP ) and related diseases along with 18 normal subjects .
	manualset3
163076	16	412129	7	NULL	NULL	0	NULL	pseudohypoparathyroidism ( PHP )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The response to exogenous parathyroid hormone ( PTH ) with urinary excretion of phosphate and cyclic adenosine monophosphate ( cAMP ) was tested by the use of synthetic human parathyroid hormone ( 1-34 ) ( hPTH - ( 1-34 ) ) on 59 patients with hypocalcemia and normal or high serum inorganic phosphorus and normal renal function without a history of parathyroidectomy for differentiation between idiopathic hypoparathyroidism ( IHP ) , pseudohypoparathyroidism ( PHP ) and related diseases along with 18 normal subjects .
	manualset3
163077	17	412129	7	NULL	NULL	NULL	NULL	 diseases	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The response to exogenous parathyroid hormone ( PTH ) with urinary excretion of phosphate and cyclic adenosine monophosphate ( cAMP ) was tested by the use of synthetic human parathyroid hormone ( 1-34 ) ( hPTH - ( 1-34 ) ) on 59 patients with hypocalcemia and normal or high serum inorganic phosphorus and normal renal function without a history of parathyroidectomy for differentiation between idiopathic hypoparathyroidism ( IHP ) , pseudohypoparathyroidism ( PHP ) and related diseases along with 18 normal subjects .
	manualset3
163078	18	412129	7	NULL	NULL	0	NULL	18 normal subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The response to exogenous parathyroid hormone ( PTH ) with urinary excretion of phosphate and cyclic adenosine monophosphate ( cAMP ) was tested by the use of synthetic human parathyroid hormone ( 1-34 ) ( hPTH - ( 1-34 ) ) on 59 patients with hypocalcemia and normal or high serum inorganic phosphorus and normal renal function without a history of parathyroidectomy for differentiation between idiopathic hypoparathyroidism ( IHP ) , pseudohypoparathyroidism ( PHP ) and related diseases along with 18 normal subjects .
	manualset3
163809	19	412129	7	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The response to exogenous parathyroid hormone ( PTH ) with urinary excretion of phosphate and cyclic adenosine monophosphate ( cAMP ) was tested by the use of synthetic human parathyroid hormone ( 1-34 ) ( hPTH - ( 1-34 ) ) on 59 patients with hypocalcemia and normal or high serum inorganic phosphorus and normal renal function without a history of parathyroidectomy for differentiation between idiopathic hypoparathyroidism ( IHP ) , pseudohypoparathyroidism ( PHP ) and related diseases along with 18 normal subjects .
	manualset3
163079	1	412130	7	NULL	NULL	0	NULL	response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The response to the attractant glucose is shown to be biphasic and perfectly adapted , as for aspartate .
	manualset3
163080	2	412130	7	NULL	NULL	0	NULL	attractant glucose	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The response to the attractant glucose is shown to be biphasic and perfectly adapted , as for aspartate .
	manualset3
163081	3	412130	7	NULL	NULL	0	NULL	biphasic 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The response to the attractant glucose is shown to be biphasic and perfectly adapted , as for aspartate .
	manualset3
163082	4	412130	7	NULL	NULL	0	NULL	aspartate	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The response to the attractant glucose is shown to be biphasic and perfectly adapted , as for aspartate .
	manualset3
163083	1	412131	7	NULL	NULL	0	NULL	 response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The response to this combination therapy is also excellent in patients who had initially responded to interferon monotherapy and later relapsed .
	manualset3
163084	2	412131	7	NULL	NULL	0	NULL	 combination therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The response to this combination therapy is also excellent in patients who had initially responded to interferon monotherapy and later relapsed .
	manualset3
163085	3	412131	7	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The response to this combination therapy is also excellent in patients who had initially responded to interferon monotherapy and later relapsed .
	manualset3
163086	4	412131	7	NULL	NULL	0	NULL	interferon monotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The response to this combination therapy is also excellent in patients who had initially responded to interferon monotherapy and later relapsed .
	manualset3
163087	1	412132	7	NULL	NULL	0	NULL	 responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The responses of soft tissue-derived prostate cancer cell lines to bone GFs and cytokines were variable .
	manualset3
163088	2	412132	7	NULL	NULL	0	NULL	soft tissue-derived prostate cancer cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The responses of soft tissue-derived prostate cancer cell lines to bone GFs and cytokines were variable .
	manualset3
163089	3	412132	7	NULL	NULL	0	NULL	bone GFs	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The responses of soft tissue-derived prostate cancer cell lines to bone GFs and cytokines were variable .
	manualset3
163090	4	412132	7	NULL	NULL	NULL	NULL	cytokines	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The responses of soft tissue-derived prostate cancer cell lines to bone GFs and cytokines were variable .
	manualset3
163091	1	412133	7	NULL	NULL	0	NULL	Abscisic acid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Abscisic acid determines basal susceptibility of tomato to Botrytis cinerea and suppresses salicylic acid-dependent signaling mechanisms .
	manualset3
163092	2	412133	7	NULL	NULL	NULL	NULL	basal susceptibility	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Abscisic acid determines basal susceptibility of tomato to Botrytis cinerea and suppresses salicylic acid-dependent signaling mechanisms .
	manualset3
163093	3	412133	7	NULL	NULL	0	NULL	tomato	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Abscisic acid determines basal susceptibility of tomato to Botrytis cinerea and suppresses salicylic acid-dependent signaling mechanisms .
	manualset3
163094	4	412133	7	NULL	NULL	0	NULL	Botrytis cinerea	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Abscisic acid determines basal susceptibility of tomato to Botrytis cinerea and suppresses salicylic acid-dependent signaling mechanisms .
	manualset3
163095	5	412133	7	NULL	NULL	0	NULL	salicylic acid-dependent signaling mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Abscisic acid determines basal susceptibility of tomato to Botrytis cinerea and suppresses salicylic acid-dependent signaling mechanisms .
	manualset3
163096	1	412134	7	NULL	NULL	0	NULL	resting NECS	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resting NECS was greater than NEA in 14 subjects with normal left ventricular end-diastolic pressure ( LVEDP ) ( p & lt ; 0.001 ) and/or in 22 with normal cardiac index ( p & lt ; 0.04 ) , whereas NECS was not significantly different from NEA in the remaining patients with elevated LVEDP and/or with reduced cardiac index .
	manualset3
163097	2	412134	7	NULL	NULL	0	NULL	 NEA	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resting NECS was greater than NEA in 14 subjects with normal left ventricular end-diastolic pressure ( LVEDP ) ( p & lt ; 0.001 ) and/or in 22 with normal cardiac index ( p & lt ; 0.04 ) , whereas NECS was not significantly different from NEA in the remaining patients with elevated LVEDP and/or with reduced cardiac index .
	manualset3
163098	3	412134	7	NULL	NULL	0	NULL	14 subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The resting NECS was greater than NEA in 14 subjects with normal left ventricular end-diastolic pressure ( LVEDP ) ( p & lt ; 0.001 ) and/or in 22 with normal cardiac index ( p & lt ; 0.04 ) , whereas NECS was not significantly different from NEA in the remaining patients with elevated LVEDP and/or with reduced cardiac index .
	manualset3
163099	4	412134	7	NULL	NULL	0	NULL	normal left ventricular end-diastolic pressure ( LVEDP )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resting NECS was greater than NEA in 14 subjects with normal left ventricular end-diastolic pressure ( LVEDP ) ( p & lt ; 0.001 ) and/or in 22 with normal cardiac index ( p & lt ; 0.04 ) , whereas NECS was not significantly different from NEA in the remaining patients with elevated LVEDP and/or with reduced cardiac index .
	manualset3
163100	5	412134	7	NULL	NULL	0	NULL	( p & lt ; 0.001 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The resting NECS was greater than NEA in 14 subjects with normal left ventricular end-diastolic pressure ( LVEDP ) ( p & lt ; 0.001 ) and/or in 22 with normal cardiac index ( p & lt ; 0.04 ) , whereas NECS was not significantly different from NEA in the remaining patients with elevated LVEDP and/or with reduced cardiac index .
	manualset3
163101	6	412134	7	NULL	NULL	0	NULL	22	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The resting NECS was greater than NEA in 14 subjects with normal left ventricular end-diastolic pressure ( LVEDP ) ( p & lt ; 0.001 ) and/or in 22 with normal cardiac index ( p & lt ; 0.04 ) , whereas NECS was not significantly different from NEA in the remaining patients with elevated LVEDP and/or with reduced cardiac index .
	manualset3
163102	7	412134	7	NULL	NULL	0	NULL	normal cardiac index 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resting NECS was greater than NEA in 14 subjects with normal left ventricular end-diastolic pressure ( LVEDP ) ( p & lt ; 0.001 ) and/or in 22 with normal cardiac index ( p & lt ; 0.04 ) , whereas NECS was not significantly different from NEA in the remaining patients with elevated LVEDP and/or with reduced cardiac index .
	manualset3
163103	8	412134	7	NULL	NULL	0	NULL	p & lt ; 0.04	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The resting NECS was greater than NEA in 14 subjects with normal left ventricular end-diastolic pressure ( LVEDP ) ( p & lt ; 0.001 ) and/or in 22 with normal cardiac index ( p & lt ; 0.04 ) , whereas NECS was not significantly different from NEA in the remaining patients with elevated LVEDP and/or with reduced cardiac index .
	manualset3
163104	9	412134	7	NULL	NULL	0	NULL	NECS	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resting NECS was greater than NEA in 14 subjects with normal left ventricular end-diastolic pressure ( LVEDP ) ( p & lt ; 0.001 ) and/or in 22 with normal cardiac index ( p & lt ; 0.04 ) , whereas NECS was not significantly different from NEA in the remaining patients with elevated LVEDP and/or with reduced cardiac index .
	manualset3
163105	10	412134	7	NULL	NULL	0	NULL	NEA	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resting NECS was greater than NEA in 14 subjects with normal left ventricular end-diastolic pressure ( LVEDP ) ( p & lt ; 0.001 ) and/or in 22 with normal cardiac index ( p & lt ; 0.04 ) , whereas NECS was not significantly different from NEA in the remaining patients with elevated LVEDP and/or with reduced cardiac index .
	manualset3
163106	11	412134	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The resting NECS was greater than NEA in 14 subjects with normal left ventricular end-diastolic pressure ( LVEDP ) ( p & lt ; 0.001 ) and/or in 22 with normal cardiac index ( p & lt ; 0.04 ) , whereas NECS was not significantly different from NEA in the remaining patients with elevated LVEDP and/or with reduced cardiac index .
	manualset3
163107	12	412134	7	NULL	NULL	0	NULL	elevated LVEDP	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resting NECS was greater than NEA in 14 subjects with normal left ventricular end-diastolic pressure ( LVEDP ) ( p & lt ; 0.001 ) and/or in 22 with normal cardiac index ( p & lt ; 0.04 ) , whereas NECS was not significantly different from NEA in the remaining patients with elevated LVEDP and/or with reduced cardiac index .
	manualset3
163108	13	412134	7	NULL	NULL	0	NULL	 reduced cardiac index	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resting NECS was greater than NEA in 14 subjects with normal left ventricular end-diastolic pressure ( LVEDP ) ( p & lt ; 0.001 ) and/or in 22 with normal cardiac index ( p & lt ; 0.04 ) , whereas NECS was not significantly different from NEA in the remaining patients with elevated LVEDP and/or with reduced cardiac index .
	manualset3
163109	1	412135	7	NULL	NULL	0	NULL	resting influx 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resting influx of 45Ca2 + into aorta rings from 7 day soman-treated and control rabbits was not different ( P greater than 0.05 ) .
	manualset3
163110	2	412135	7	NULL	NULL	0	NULL	45Ca2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The resting influx of 45Ca2 + into aorta rings from 7 day soman-treated and control rabbits was not different ( P greater than 0.05 ) .
	manualset3
163111	3	412135	7	NULL	NULL	0	NULL	aorta rings 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The resting influx of 45Ca2 + into aorta rings from 7 day soman-treated and control rabbits was not different ( P greater than 0.05 ) .
	manualset3
163112	4	412135	7	NULL	NULL	0	NULL	7 day	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The resting influx of 45Ca2 + into aorta rings from 7 day soman-treated and control rabbits was not different ( P greater than 0.05 ) .
	manualset3
163113	5	412135	7	NULL	NULL	0	NULL	soman-treated rabbits	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The resting influx of 45Ca2 + into aorta rings from 7 day soman-treated and control rabbits was not different ( P greater than 0.05 ) .
	manualset3
163114	6	412135	7	NULL	NULL	0	NULL	control rabbits	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The resting influx of 45Ca2 + into aorta rings from 7 day soman-treated and control rabbits was not different ( P greater than 0.05 ) .
	manualset3
163115	7	412135	7	NULL	NULL	0	NULL	P greater than 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The resting influx of 45Ca2 + into aorta rings from 7 day soman-treated and control rabbits was not different ( P greater than 0.05 ) .
	manualset3
163116	1	412136	7	NULL	NULL	0	NULL	restored FRAP activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The restored FRAP activity therefore reflects renewed synthesis and transport of enzyme in still injured neurons , and not central sprouting of intact neighboring afferents .
	manualset3
163117	2	412136	7	NULL	NULL	0	NULL	 synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The restored FRAP activity therefore reflects renewed synthesis and transport of enzyme in still injured neurons , and not central sprouting of intact neighboring afferents .
	manualset3
163118	3	412136	7	NULL	NULL	NULL	NULL	transport of enzyme	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The restored FRAP activity therefore reflects renewed synthesis and transport of enzyme in still injured neurons , and not central sprouting of intact neighboring afferents .
	manualset3
163119	4	412136	7	NULL	NULL	NULL	NULL	 injured neurons	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The restored FRAP activity therefore reflects renewed synthesis and transport of enzyme in still injured neurons , and not central sprouting of intact neighboring afferents .
	manualset3
163120	5	412136	7	NULL	NULL	0	NULL	central sprouting	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The restored FRAP activity therefore reflects renewed synthesis and transport of enzyme in still injured neurons , and not central sprouting of intact neighboring afferents .
	manualset3
163121	6	412136	7	NULL	NULL	0	NULL	intact neighboring afferents	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The restored FRAP activity therefore reflects renewed synthesis and transport of enzyme in still injured neurons , and not central sprouting of intact neighboring afferents .
	manualset3
163123	1	412137	7	NULL	NULL	0	NULL	facultative methylotrophs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The restricted facultative methylotrophs grow on certain non-C1 compounds in the absence of 2-oxoglutarate dehydrogenase and , in some cases , of other enzymes of the tricarboxylic acid cycle ; these lesions can not therefore be the sole cause of obligate methylotrophy .
	manualset3
163124	2	412137	7	NULL	NULL	0	NULL	non-C1 compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The restricted facultative methylotrophs grow on certain non-C1 compounds in the absence of 2-oxoglutarate dehydrogenase and , in some cases , of other enzymes of the tricarboxylic acid cycle ; these lesions can not therefore be the sole cause of obligate methylotrophy .
	manualset3
163125	3	412137	7	NULL	NULL	NULL	NULL	absence	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The restricted facultative methylotrophs grow on certain non-C1 compounds in the absence of 2-oxoglutarate dehydrogenase and , in some cases , of other enzymes of the tricarboxylic acid cycle ; these lesions can not therefore be the sole cause of obligate methylotrophy .
	manualset3
163126	4	412137	7	NULL	NULL	0	NULL	2-oxoglutarate dehydrogenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The restricted facultative methylotrophs grow on certain non-C1 compounds in the absence of 2-oxoglutarate dehydrogenase and , in some cases , of other enzymes of the tricarboxylic acid cycle ; these lesions can not therefore be the sole cause of obligate methylotrophy .
	manualset3
163128	6	412137	7	NULL	NULL	0	NULL	enzymes	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The restricted facultative methylotrophs grow on certain non-C1 compounds in the absence of 2-oxoglutarate dehydrogenase and , in some cases , of other enzymes of the tricarboxylic acid cycle ; these lesions can not therefore be the sole cause of obligate methylotrophy .
	manualset3
163129	7	412137	7	NULL	NULL	0	NULL	tricarboxylic acid cycle 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The restricted facultative methylotrophs grow on certain non-C1 compounds in the absence of 2-oxoglutarate dehydrogenase and , in some cases , of other enzymes of the tricarboxylic acid cycle ; these lesions can not therefore be the sole cause of obligate methylotrophy .
	manualset3
163130	8	412137	7	NULL	NULL	NULL	NULL	lesions	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The restricted facultative methylotrophs grow on certain non-C1 compounds in the absence of 2-oxoglutarate dehydrogenase and , in some cases , of other enzymes of the tricarboxylic acid cycle ; these lesions can not therefore be the sole cause of obligate methylotrophy .
	manualset3
163131	9	412137	7	NULL	NULL	NULL	NULL	cause	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The restricted facultative methylotrophs grow on certain non-C1 compounds in the absence of 2-oxoglutarate dehydrogenase and , in some cases , of other enzymes of the tricarboxylic acid cycle ; these lesions can not therefore be the sole cause of obligate methylotrophy .
	manualset3
163132	10	412137	7	NULL	NULL	NULL	NULL	obligate methylotrophy	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The restricted facultative methylotrophs grow on certain non-C1 compounds in the absence of 2-oxoglutarate dehydrogenase and , in some cases , of other enzymes of the tricarboxylic acid cycle ; these lesions can not therefore be the sole cause of obligate methylotrophy .
	manualset3
169726	11	412137	7	NULL	NULL	0	NULL	cases	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The restricted facultative methylotrophs grow on certain non-C1 compounds in the absence of 2-oxoglutarate dehydrogenase and , in some cases , of other enzymes of the tricarboxylic acid cycle ; these lesions can not therefore be the sole cause of obligate methylotrophy .
	manualset3
163133	1	412138	7	NULL	NULL	0	NULL	 range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The restricted range of the species pairs places them at risk of extinction , and one of the pairs has gone extinct after the introduction of an exotic catfish .
	manualset3
163134	2	412138	7	NULL	NULL	NULL	NULL	 species pairs	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The restricted range of the species pairs places them at risk of extinction , and one of the pairs has gone extinct after the introduction of an exotic catfish .
	manualset3
163135	3	412138	7	NULL	NULL	NULL	NULL	 risk 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The restricted range of the species pairs places them at risk of extinction , and one of the pairs has gone extinct after the introduction of an exotic catfish .
	manualset3
163136	4	412138	7	NULL	NULL	0	NULL	extinction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The restricted range of the species pairs places them at risk of extinction , and one of the pairs has gone extinct after the introduction of an exotic catfish .
	manualset3
163137	5	412138	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The restricted range of the species pairs places them at risk of extinction , and one of the pairs has gone extinct after the introduction of an exotic catfish .
	manualset3
163138	6	412138	7	NULL	NULL	0	NULL	pairs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The restricted range of the species pairs places them at risk of extinction , and one of the pairs has gone extinct after the introduction of an exotic catfish .
	manualset3
163139	7	412138	7	NULL	NULL	0	NULL	 introduction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The restricted range of the species pairs places them at risk of extinction , and one of the pairs has gone extinct after the introduction of an exotic catfish .
	manualset3
163140	8	412138	7	NULL	NULL	0	NULL	exotic catfish	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The restricted range of the species pairs places them at risk of extinction , and one of the pairs has gone extinct after the introduction of an exotic catfish .
	manualset3
163141	1	412139	7	NULL	NULL	0	NULL	restriction enzyme patterns 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The restriction enzyme patterns of HPRS 24 ( serotype 2 ) differed substantially from those of HPRS 16 and HPRS 16/att and reassociation experiments showed that HPRS 24 shares less than 10 % homology with either HPRS 16 or herpesvirus of turkeys ( serotype 3 ) .
	manualset3
163142	2	412139	7	NULL	NULL	NULL	NULL	HPRS 24 ( serotype 2 )	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The restriction enzyme patterns of HPRS 24 ( serotype 2 ) differed substantially from those of HPRS 16 and HPRS 16/att and reassociation experiments showed that HPRS 24 shares less than 10 % homology with either HPRS 16 or herpesvirus of turkeys ( serotype 3 ) .
	manualset3
163143	3	412139	7	NULL	NULL	NULL	NULL	HPRS 16	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The restriction enzyme patterns of HPRS 24 ( serotype 2 ) differed substantially from those of HPRS 16 and HPRS 16/att and reassociation experiments showed that HPRS 24 shares less than 10 % homology with either HPRS 16 or herpesvirus of turkeys ( serotype 3 ) .
	manualset3
163144	4	412139	7	NULL	NULL	NULL	NULL	HPRS 16/att 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The restriction enzyme patterns of HPRS 24 ( serotype 2 ) differed substantially from those of HPRS 16 and HPRS 16/att and reassociation experiments showed that HPRS 24 shares less than 10 % homology with either HPRS 16 or herpesvirus of turkeys ( serotype 3 ) .
	manualset3
163145	5	412139	7	NULL	NULL	0	NULL	reassociation experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The restriction enzyme patterns of HPRS 24 ( serotype 2 ) differed substantially from those of HPRS 16 and HPRS 16/att and reassociation experiments showed that HPRS 24 shares less than 10 % homology with either HPRS 16 or herpesvirus of turkeys ( serotype 3 ) .
	manualset3
163146	6	412139	7	NULL	NULL	NULL	NULL	HPRS 24 ( serotype 2 )	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The restriction enzyme patterns of HPRS 24 ( serotype 2 ) differed substantially from those of HPRS 16 and HPRS 16/att and reassociation experiments showed that HPRS 24 shares less than 10 % homology with either HPRS 16 or herpesvirus of turkeys ( serotype 3 ) .
	manualset3
163147	7	412139	7	NULL	NULL	0	NULL	10 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The restriction enzyme patterns of HPRS 24 ( serotype 2 ) differed substantially from those of HPRS 16 and HPRS 16/att and reassociation experiments showed that HPRS 24 shares less than 10 % homology with either HPRS 16 or herpesvirus of turkeys ( serotype 3 ) .
	manualset3
163148	8	412139	7	NULL	NULL	NULL	NULL	homology 	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The restriction enzyme patterns of HPRS 24 ( serotype 2 ) differed substantially from those of HPRS 16 and HPRS 16/att and reassociation experiments showed that HPRS 24 shares less than 10 % homology with either HPRS 16 or herpesvirus of turkeys ( serotype 3 ) .
	manualset3
163149	9	412139	7	NULL	NULL	0	NULL	HPRS 16	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The restriction enzyme patterns of HPRS 24 ( serotype 2 ) differed substantially from those of HPRS 16 and HPRS 16/att and reassociation experiments showed that HPRS 24 shares less than 10 % homology with either HPRS 16 or herpesvirus of turkeys ( serotype 3 ) .
	manualset3
163150	10	412139	7	NULL	NULL	0	NULL	herpesvirus of turkeys ( serotype 3 ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The restriction enzyme patterns of HPRS 24 ( serotype 2 ) differed substantially from those of HPRS 16 and HPRS 16/att and reassociation experiments showed that HPRS 24 shares less than 10 % homology with either HPRS 16 or herpesvirus of turkeys ( serotype 3 ) .
	manualset3
163151	1	412140	7	NULL	NULL	NULL	NULL	result 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The result revealed , for the first time , two different courses of deficient cervical kinaesthesia .
	manualset3
163152	2	412140	7	NULL	NULL	0	NULL	first time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The result revealed , for the first time , two different courses of deficient cervical kinaesthesia .
	manualset3
163153	3	412140	7	NULL	NULL	0	NULL	 two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The result revealed , for the first time , two different courses of deficient cervical kinaesthesia .
	manualset3
163154	4	412140	7	NULL	NULL	0	NULL	courses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The result revealed , for the first time , two different courses of deficient cervical kinaesthesia .
	manualset3
163155	5	412140	7	NULL	NULL	0	NULL	deficient cervical kinaesthesia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The result revealed , for the first time , two different courses of deficient cervical kinaesthesia .
	manualset3
163156	1	412141	7	NULL	NULL	NULL	NULL	result	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The result revealed that the ME1-Dra I genotypes had a significant effect on cooking loss , pH measured 24h post-mortem ( pH ( 24h ) ) and eye muscle area ( P & lt ; 0.05 ) .
	manualset3
163157	2	412141	7	NULL	NULL	0	NULL	ME1-Dra I genotypes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The result revealed that the ME1-Dra I genotypes had a significant effect on cooking loss , pH measured 24h post-mortem ( pH ( 24h ) ) and eye muscle area ( P & lt ; 0.05 ) .
	manualset3
163158	3	412141	7	NULL	NULL	0	NULL	cooking loss	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The result revealed that the ME1-Dra I genotypes had a significant effect on cooking loss , pH measured 24h post-mortem ( pH ( 24h ) ) and eye muscle area ( P & lt ; 0.05 ) .
	manualset3
163159	4	412141	7	NULL	NULL	0	NULL	 pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The result revealed that the ME1-Dra I genotypes had a significant effect on cooking loss , pH measured 24h post-mortem ( pH ( 24h ) ) and eye muscle area ( P & lt ; 0.05 ) .
	manualset3
163160	5	412141	7	NULL	NULL	0	NULL	24h post-mortem	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The result revealed that the ME1-Dra I genotypes had a significant effect on cooking loss , pH measured 24h post-mortem ( pH ( 24h ) ) and eye muscle area ( P & lt ; 0.05 ) .
	manualset3
163161	6	412141	7	NULL	NULL	0	NULL	pH ( 24h )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The result revealed that the ME1-Dra I genotypes had a significant effect on cooking loss , pH measured 24h post-mortem ( pH ( 24h ) ) and eye muscle area ( P & lt ; 0.05 ) .
	manualset3
163162	7	412141	7	NULL	NULL	0	NULL	eye muscle area	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The result revealed that the ME1-Dra I genotypes had a significant effect on cooking loss , pH measured 24h post-mortem ( pH ( 24h ) ) and eye muscle area ( P & lt ; 0.05 ) .
	manualset3
163163	8	412141	7	NULL	NULL	0	NULL	P & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The result revealed that the ME1-Dra I genotypes had a significant effect on cooking loss , pH measured 24h post-mortem ( pH ( 24h ) ) and eye muscle area ( P & lt ; 0.05 ) .
	manualset3
163164	1	412142	7	NULL	NULL	NULL	NULL	result 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The result showed that PSP is composed of fructose only .
	manualset3
163165	2	412142	7	NULL	NULL	0	NULL	PSP	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The result showed that PSP is composed of fructose only .
	manualset3
163166	3	412142	7	NULL	NULL	0	NULL	fructose	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The result showed that PSP is composed of fructose only .
	manualset3
163167	1	412143	7	NULL	NULL	0	NULL	Absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Absence of HTLV-I DNA in blood from patients with multiple sclerosis .
	manualset3
163168	2	412143	7	NULL	NULL	0	NULL	HTLV-I DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Absence of HTLV-I DNA in blood from patients with multiple sclerosis .
	manualset3
163169	3	412143	7	NULL	NULL	0	NULL	blood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Absence of HTLV-I DNA in blood from patients with multiple sclerosis .
	manualset3
163170	4	412143	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Absence of HTLV-I DNA in blood from patients with multiple sclerosis .
	manualset3
163171	5	412143	7	NULL	NULL	0	NULL	multiple sclerosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Absence of HTLV-I DNA in blood from patients with multiple sclerosis .
	manualset3
163172	1	412144	7	NULL	NULL	NULL	NULL	 result 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The result showed that all but Cg could inhibit lipid peroxidation .
	manualset3
163173	2	412144	7	NULL	NULL	0	NULL	Cg	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The result showed that all but Cg could inhibit lipid peroxidation .
	manualset3
163174	3	412144	7	NULL	NULL	NULL	NULL	lipid peroxidation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The result showed that all but Cg could inhibit lipid peroxidation .
	manualset3
163175	1	412145	7	NULL	NULL	NULL	NULL	result	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The result showed the SNP-819C / T was significantly correlated with Deficiency syndrome ( P = 0.031 ) , but none of the 3 loci showed correlation either with Child-Pugh classification and phase in HBC patients .
	manualset3
163176	2	412145	7	NULL	NULL	0	NULL	SNP-819C / T	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The result showed the SNP-819C / T was significantly correlated with Deficiency syndrome ( P = 0.031 ) , but none of the 3 loci showed correlation either with Child-Pugh classification and phase in HBC patients .
	manualset3
163177	3	412145	7	NULL	NULL	0	NULL	Deficiency syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The result showed the SNP-819C / T was significantly correlated with Deficiency syndrome ( P = 0.031 ) , but none of the 3 loci showed correlation either with Child-Pugh classification and phase in HBC patients .
	manualset3
163178	4	412145	7	NULL	NULL	0	NULL	P = 0.031	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The result showed the SNP-819C / T was significantly correlated with Deficiency syndrome ( P = 0.031 ) , but none of the 3 loci showed correlation either with Child-Pugh classification and phase in HBC patients .
	manualset3
163179	5	412145	7	NULL	NULL	0	NULL	 3 loci	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The result showed the SNP-819C / T was significantly correlated with Deficiency syndrome ( P = 0.031 ) , but none of the 3 loci showed correlation either with Child-Pugh classification and phase in HBC patients .
	manualset3
163180	6	412145	7	NULL	NULL	0	NULL	Child-Pugh classification	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The result showed the SNP-819C / T was significantly correlated with Deficiency syndrome ( P = 0.031 ) , but none of the 3 loci showed correlation either with Child-Pugh classification and phase in HBC patients .
	manualset3
163181	7	412145	7	NULL	NULL	0	NULL	phase	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The result showed the SNP-819C / T was significantly correlated with Deficiency syndrome ( P = 0.031 ) , but none of the 3 loci showed correlation either with Child-Pugh classification and phase in HBC patients .
	manualset3
163182	8	412145	7	NULL	NULL	0	NULL	HBC patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The result showed the SNP-819C / T was significantly correlated with Deficiency syndrome ( P = 0.031 ) , but none of the 3 loci showed correlation either with Child-Pugh classification and phase in HBC patients .
	manualset3
164580	9	412145	7	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The result showed the SNP-819C / T was significantly correlated with Deficiency syndrome ( P = 0.031 ) , but none of the 3 loci showed correlation either with Child-Pugh classification and phase in HBC patients .
	manualset3
163183	1	412146	7	NULL	NULL	NULL	NULL	result 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The result was good for thirty-one ankles ( 19 per cent ) , fair for fifty-five ( 34 per cent ) , and poor for seventeen ( 11 per cent ) ; fifty-seven arthroplasties ( 36 per cent ) were considered to be a failure ( defined as removal of the implant ) .
	manualset3
163184	2	412146	7	NULL	NULL	0	NULL	thirty-one ankles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The result was good for thirty-one ankles ( 19 per cent ) , fair for fifty-five ( 34 per cent ) , and poor for seventeen ( 11 per cent ) ; fifty-seven arthroplasties ( 36 per cent ) were considered to be a failure ( defined as removal of the implant ) .
	manualset3
163185	3	412146	7	NULL	NULL	0	NULL	19 per cent	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The result was good for thirty-one ankles ( 19 per cent ) , fair for fifty-five ( 34 per cent ) , and poor for seventeen ( 11 per cent ) ; fifty-seven arthroplasties ( 36 per cent ) were considered to be a failure ( defined as removal of the implant ) .
	manualset3
163186	4	412146	7	NULL	NULL	0	NULL	 fifty-five	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The result was good for thirty-one ankles ( 19 per cent ) , fair for fifty-five ( 34 per cent ) , and poor for seventeen ( 11 per cent ) ; fifty-seven arthroplasties ( 36 per cent ) were considered to be a failure ( defined as removal of the implant ) .
	manualset3
163187	5	412146	7	NULL	NULL	0	NULL	 34 per cent 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The result was good for thirty-one ankles ( 19 per cent ) , fair for fifty-five ( 34 per cent ) , and poor for seventeen ( 11 per cent ) ; fifty-seven arthroplasties ( 36 per cent ) were considered to be a failure ( defined as removal of the implant ) .
	manualset3
163188	6	412146	7	NULL	NULL	0	NULL	 seventeen	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The result was good for thirty-one ankles ( 19 per cent ) , fair for fifty-five ( 34 per cent ) , and poor for seventeen ( 11 per cent ) ; fifty-seven arthroplasties ( 36 per cent ) were considered to be a failure ( defined as removal of the implant ) .
	manualset3
163189	7	412146	7	NULL	NULL	0	NULL	11 per cent	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The result was good for thirty-one ankles ( 19 per cent ) , fair for fifty-five ( 34 per cent ) , and poor for seventeen ( 11 per cent ) ; fifty-seven arthroplasties ( 36 per cent ) were considered to be a failure ( defined as removal of the implant ) .
	manualset3
163190	8	412146	7	NULL	NULL	0	NULL	 fifty-seven	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The result was good for thirty-one ankles ( 19 per cent ) , fair for fifty-five ( 34 per cent ) , and poor for seventeen ( 11 per cent ) ; fifty-seven arthroplasties ( 36 per cent ) were considered to be a failure ( defined as removal of the implant ) .
	manualset3
163191	9	412146	7	NULL	NULL	0	NULL	arthroplasties	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The result was good for thirty-one ankles ( 19 per cent ) , fair for fifty-five ( 34 per cent ) , and poor for seventeen ( 11 per cent ) ; fifty-seven arthroplasties ( 36 per cent ) were considered to be a failure ( defined as removal of the implant ) .
	manualset3
163192	10	412146	7	NULL	NULL	0	NULL	36 per cent	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The result was good for thirty-one ankles ( 19 per cent ) , fair for fifty-five ( 34 per cent ) , and poor for seventeen ( 11 per cent ) ; fifty-seven arthroplasties ( 36 per cent ) were considered to be a failure ( defined as removal of the implant ) .
	manualset3
163193	11	412146	7	NULL	NULL	0	NULL	 failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The result was good for thirty-one ankles ( 19 per cent ) , fair for fifty-five ( 34 per cent ) , and poor for seventeen ( 11 per cent ) ; fifty-seven arthroplasties ( 36 per cent ) were considered to be a failure ( defined as removal of the implant ) .
	manualset3
163194	12	412146	7	NULL	NULL	NULL	NULL	removal	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The result was good for thirty-one ankles ( 19 per cent ) , fair for fifty-five ( 34 per cent ) , and poor for seventeen ( 11 per cent ) ; fifty-seven arthroplasties ( 36 per cent ) were considered to be a failure ( defined as removal of the implant ) .
	manualset3
163247	13	412146	7	NULL	NULL	0	NULL	implant	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The result was good for thirty-one ankles ( 19 per cent ) , fair for fifty-five ( 34 per cent ) , and poor for seventeen ( 11 per cent ) ; fifty-seven arthroplasties ( 36 per cent ) were considered to be a failure ( defined as removal of the implant ) .
	manualset3
163195	1	412147	7	NULL	NULL	0	NULL	2 , 019-bp partial sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The resultant 2 , 019-bp partial sequence of the DNA polymerase gene of the newfound herpesvirus , including the original 483-bp region , showed a high degree of homology at both the nucleotide and amino acid levels with that of other human and animal herpesviruses .
	manualset3
163196	2	412147	7	NULL	NULL	0	NULL	DNA polymerase gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The resultant 2 , 019-bp partial sequence of the DNA polymerase gene of the newfound herpesvirus , including the original 483-bp region , showed a high degree of homology at both the nucleotide and amino acid levels with that of other human and animal herpesviruses .
	manualset3
163197	3	412147	7	NULL	NULL	0	NULL	herpesvirus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The resultant 2 , 019-bp partial sequence of the DNA polymerase gene of the newfound herpesvirus , including the original 483-bp region , showed a high degree of homology at both the nucleotide and amino acid levels with that of other human and animal herpesviruses .
	manualset3
163198	4	412147	7	NULL	NULL	0	NULL	483-bp region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The resultant 2 , 019-bp partial sequence of the DNA polymerase gene of the newfound herpesvirus , including the original 483-bp region , showed a high degree of homology at both the nucleotide and amino acid levels with that of other human and animal herpesviruses .
	manualset3
163199	5	412147	7	NULL	NULL	0	NULL	high degree	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resultant 2 , 019-bp partial sequence of the DNA polymerase gene of the newfound herpesvirus , including the original 483-bp region , showed a high degree of homology at both the nucleotide and amino acid levels with that of other human and animal herpesviruses .
	manualset3
163200	6	412147	7	NULL	NULL	0	NULL	homology	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The resultant 2 , 019-bp partial sequence of the DNA polymerase gene of the newfound herpesvirus , including the original 483-bp region , showed a high degree of homology at both the nucleotide and amino acid levels with that of other human and animal herpesviruses .
	manualset3
163201	7	412147	7	NULL	NULL	0	NULL	nucleotide	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The resultant 2 , 019-bp partial sequence of the DNA polymerase gene of the newfound herpesvirus , including the original 483-bp region , showed a high degree of homology at both the nucleotide and amino acid levels with that of other human and animal herpesviruses .
	manualset3
163202	8	412147	7	NULL	NULL	NULL	NULL	amino acid levels	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The resultant 2 , 019-bp partial sequence of the DNA polymerase gene of the newfound herpesvirus , including the original 483-bp region , showed a high degree of homology at both the nucleotide and amino acid levels with that of other human and animal herpesviruses .
	manualset3
163203	9	412147	7	NULL	NULL	0	NULL	 human herspesvirus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The resultant 2 , 019-bp partial sequence of the DNA polymerase gene of the newfound herpesvirus , including the original 483-bp region , showed a high degree of homology at both the nucleotide and amino acid levels with that of other human and animal herpesviruses .
	manualset3
163204	10	412147	7	NULL	NULL	0	NULL	animal herpesviruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The resultant 2 , 019-bp partial sequence of the DNA polymerase gene of the newfound herpesvirus , including the original 483-bp region , showed a high degree of homology at both the nucleotide and amino acid levels with that of other human and animal herpesviruses .
	manualset3
163205	1	412148	7	NULL	NULL	0	NULL	 resultant strains 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The resultant strains included a mutant in which Env residue 767 was changed to a stop codon , a double mutant in which positions 738 and 739 were changed to stop codons , another mutant in which a prominent endocytosis motif was changed from YRPV to GRPV by the substitution of tyrosine 721 , and a final combination mutant bearing Q738stop , Q739stop , and Y721G mutations .
	manualset3
163206	2	412148	7	NULL	NULL	NULL	NULL	mutant	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The resultant strains included a mutant in which Env residue 767 was changed to a stop codon , a double mutant in which positions 738 and 739 were changed to stop codons , another mutant in which a prominent endocytosis motif was changed from YRPV to GRPV by the substitution of tyrosine 721 , and a final combination mutant bearing Q738stop , Q739stop , and Y721G mutations .
	manualset3
163207	3	412148	7	NULL	NULL	0	NULL	Env residue 767	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The resultant strains included a mutant in which Env residue 767 was changed to a stop codon , a double mutant in which positions 738 and 739 were changed to stop codons , another mutant in which a prominent endocytosis motif was changed from YRPV to GRPV by the substitution of tyrosine 721 , and a final combination mutant bearing Q738stop , Q739stop , and Y721G mutations .
	manualset3
163208	4	412148	7	NULL	NULL	0	NULL	stop codon	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The resultant strains included a mutant in which Env residue 767 was changed to a stop codon , a double mutant in which positions 738 and 739 were changed to stop codons , another mutant in which a prominent endocytosis motif was changed from YRPV to GRPV by the substitution of tyrosine 721 , and a final combination mutant bearing Q738stop , Q739stop , and Y721G mutations .
	manualset3
163209	5	412148	7	NULL	NULL	NULL	NULL	double mutant	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The resultant strains included a mutant in which Env residue 767 was changed to a stop codon , a double mutant in which positions 738 and 739 were changed to stop codons , another mutant in which a prominent endocytosis motif was changed from YRPV to GRPV by the substitution of tyrosine 721 , and a final combination mutant bearing Q738stop , Q739stop , and Y721G mutations .
	manualset3
163210	6	412148	7	NULL	NULL	0	NULL	positions 738	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resultant strains included a mutant in which Env residue 767 was changed to a stop codon , a double mutant in which positions 738 and 739 were changed to stop codons , another mutant in which a prominent endocytosis motif was changed from YRPV to GRPV by the substitution of tyrosine 721 , and a final combination mutant bearing Q738stop , Q739stop , and Y721G mutations .
	manualset3
163211	7	412148	7	NULL	NULL	0	NULL	positions 739	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resultant strains included a mutant in which Env residue 767 was changed to a stop codon , a double mutant in which positions 738 and 739 were changed to stop codons , another mutant in which a prominent endocytosis motif was changed from YRPV to GRPV by the substitution of tyrosine 721 , and a final combination mutant bearing Q738stop , Q739stop , and Y721G mutations .
	manualset3
163212	8	412148	7	NULL	NULL	0	NULL	stop codons	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The resultant strains included a mutant in which Env residue 767 was changed to a stop codon , a double mutant in which positions 738 and 739 were changed to stop codons , another mutant in which a prominent endocytosis motif was changed from YRPV to GRPV by the substitution of tyrosine 721 , and a final combination mutant bearing Q738stop , Q739stop , and Y721G mutations .
	manualset3
163213	9	412148	7	NULL	NULL	NULL	NULL	mutant	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The resultant strains included a mutant in which Env residue 767 was changed to a stop codon , a double mutant in which positions 738 and 739 were changed to stop codons , another mutant in which a prominent endocytosis motif was changed from YRPV to GRPV by the substitution of tyrosine 721 , and a final combination mutant bearing Q738stop , Q739stop , and Y721G mutations .
	manualset3
163214	10	412148	7	NULL	NULL	0	NULL	endocytosis motif	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resultant strains included a mutant in which Env residue 767 was changed to a stop codon , a double mutant in which positions 738 and 739 were changed to stop codons , another mutant in which a prominent endocytosis motif was changed from YRPV to GRPV by the substitution of tyrosine 721 , and a final combination mutant bearing Q738stop , Q739stop , and Y721G mutations .
	manualset3
163215	11	412148	7	NULL	NULL	0	NULL	YRPV	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The resultant strains included a mutant in which Env residue 767 was changed to a stop codon , a double mutant in which positions 738 and 739 were changed to stop codons , another mutant in which a prominent endocytosis motif was changed from YRPV to GRPV by the substitution of tyrosine 721 , and a final combination mutant bearing Q738stop , Q739stop , and Y721G mutations .
	manualset3
163216	12	412148	7	NULL	NULL	0	NULL	GRPV	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The resultant strains included a mutant in which Env residue 767 was changed to a stop codon , a double mutant in which positions 738 and 739 were changed to stop codons , another mutant in which a prominent endocytosis motif was changed from YRPV to GRPV by the substitution of tyrosine 721 , and a final combination mutant bearing Q738stop , Q739stop , and Y721G mutations .
	manualset3
163217	13	412148	7	NULL	NULL	NULL	NULL	 substitution	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The resultant strains included a mutant in which Env residue 767 was changed to a stop codon , a double mutant in which positions 738 and 739 were changed to stop codons , another mutant in which a prominent endocytosis motif was changed from YRPV to GRPV by the substitution of tyrosine 721 , and a final combination mutant bearing Q738stop , Q739stop , and Y721G mutations .
	manualset3
163218	14	412148	7	NULL	NULL	0	NULL	tyrosine 721	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The resultant strains included a mutant in which Env residue 767 was changed to a stop codon , a double mutant in which positions 738 and 739 were changed to stop codons , another mutant in which a prominent endocytosis motif was changed from YRPV to GRPV by the substitution of tyrosine 721 , and a final combination mutant bearing Q738stop , Q739stop , and Y721G mutations .
	manualset3
163219	15	412148	7	NULL	NULL	0	NULL	combination mutant 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The resultant strains included a mutant in which Env residue 767 was changed to a stop codon , a double mutant in which positions 738 and 739 were changed to stop codons , another mutant in which a prominent endocytosis motif was changed from YRPV to GRPV by the substitution of tyrosine 721 , and a final combination mutant bearing Q738stop , Q739stop , and Y721G mutations .
	manualset3
163220	16	412148	7	NULL	NULL	0	NULL	Q738stop	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The resultant strains included a mutant in which Env residue 767 was changed to a stop codon , a double mutant in which positions 738 and 739 were changed to stop codons , another mutant in which a prominent endocytosis motif was changed from YRPV to GRPV by the substitution of tyrosine 721 , and a final combination mutant bearing Q738stop , Q739stop , and Y721G mutations .
	manualset3
163221	17	412148	7	NULL	NULL	0	NULL	Q739stop	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The resultant strains included a mutant in which Env residue 767 was changed to a stop codon , a double mutant in which positions 738 and 739 were changed to stop codons , another mutant in which a prominent endocytosis motif was changed from YRPV to GRPV by the substitution of tyrosine 721 , and a final combination mutant bearing Q738stop , Q739stop , and Y721G mutations .
	manualset3
163222	18	412148	7	NULL	NULL	NULL	NULL	Y721G mutations	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The resultant strains included a mutant in which Env residue 767 was changed to a stop codon , a double mutant in which positions 738 and 739 were changed to stop codons , another mutant in which a prominent endocytosis motif was changed from YRPV to GRPV by the substitution of tyrosine 721 , and a final combination mutant bearing Q738stop , Q739stop , and Y721G mutations .
	manualset3
163223	1	412149	7	NULL	NULL	0	NULL	HOX11 gene expression signature	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting HOX11 gene expression signature , which was validated for representative signaling pathways by transient transfection of reporter constructs , was characterized by elevated expression of transcriptional programs involved in cell proliferation , including those regulated by E2F , c-Myc and cAMP response element-binding protein .
	manualset3
163224	2	412149	7	NULL	NULL	0	NULL	signaling pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting HOX11 gene expression signature , which was validated for representative signaling pathways by transient transfection of reporter constructs , was characterized by elevated expression of transcriptional programs involved in cell proliferation , including those regulated by E2F , c-Myc and cAMP response element-binding protein .
	manualset3
163225	3	412149	7	NULL	NULL	NULL	NULL	transient transfection of reporter constructs	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The resulting HOX11 gene expression signature , which was validated for representative signaling pathways by transient transfection of reporter constructs , was characterized by elevated expression of transcriptional programs involved in cell proliferation , including those regulated by E2F , c-Myc and cAMP response element-binding protein .
	manualset3
163227	5	412149	7	NULL	NULL	0	NULL	elevated expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting HOX11 gene expression signature , which was validated for representative signaling pathways by transient transfection of reporter constructs , was characterized by elevated expression of transcriptional programs involved in cell proliferation , including those regulated by E2F , c-Myc and cAMP response element-binding protein .
	manualset3
163228	6	412149	7	NULL	NULL	0	NULL	transcriptional programs	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting HOX11 gene expression signature , which was validated for representative signaling pathways by transient transfection of reporter constructs , was characterized by elevated expression of transcriptional programs involved in cell proliferation , including those regulated by E2F , c-Myc and cAMP response element-binding protein .
	manualset3
163229	7	412149	7	NULL	NULL	NULL	NULL	cell proliferation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The resulting HOX11 gene expression signature , which was validated for representative signaling pathways by transient transfection of reporter constructs , was characterized by elevated expression of transcriptional programs involved in cell proliferation , including those regulated by E2F , c-Myc and cAMP response element-binding protein .
	manualset3
163230	8	412149	7	NULL	NULL	0	NULL	E2F	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting HOX11 gene expression signature , which was validated for representative signaling pathways by transient transfection of reporter constructs , was characterized by elevated expression of transcriptional programs involved in cell proliferation , including those regulated by E2F , c-Myc and cAMP response element-binding protein .
	manualset3
163231	9	412149	7	NULL	NULL	0	NULL	c-Myc 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting HOX11 gene expression signature , which was validated for representative signaling pathways by transient transfection of reporter constructs , was characterized by elevated expression of transcriptional programs involved in cell proliferation , including those regulated by E2F , c-Myc and cAMP response element-binding protein .
	manualset3
163232	10	412149	7	NULL	NULL	0	NULL	cAMP response element-binding protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting HOX11 gene expression signature , which was validated for representative signaling pathways by transient transfection of reporter constructs , was characterized by elevated expression of transcriptional programs involved in cell proliferation , including those regulated by E2F , c-Myc and cAMP response element-binding protein .
	manualset3
163233	1	412150	7	NULL	NULL	0	NULL	IAM-HLADH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting IAM-HLADH retained the reductive activity of native HLADH as well as the enzyme 's enantioselectivity and enantiospecificity .
	manualset3
163234	2	412150	7	NULL	NULL	NULL	NULL	reductive activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The resulting IAM-HLADH retained the reductive activity of native HLADH as well as the enzyme 's enantioselectivity and enantiospecificity .
	manualset3
163235	3	412150	7	NULL	NULL	0	NULL	native HLADH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting IAM-HLADH retained the reductive activity of native HLADH as well as the enzyme 's enantioselectivity and enantiospecificity .
	manualset3
163236	4	412150	7	NULL	NULL	NULL	NULL	enzyme 's enantioselectivity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The resulting IAM-HLADH retained the reductive activity of native HLADH as well as the enzyme 's enantioselectivity and enantiospecificity .
	manualset3
163237	5	412150	7	NULL	NULL	NULL	NULL	enantiospecificity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The resulting IAM-HLADH retained the reductive activity of native HLADH as well as the enzyme 's enantioselectivity and enantiospecificity .
	manualset3
163238	1	412151	7	NULL	NULL	0	NULL	stochastic fraction 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting `` stochastic fraction '' ( tumors for which treatment outcome is probabilistic ) would be characterized by a steep dose response , and the number of patients required to demonstrate the effect of dose escalation would be substantially reduced ( by about 50 % ) .
	manualset3
163239	2	412151	7	NULL	NULL	0	NULL	tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting `` stochastic fraction '' ( tumors for which treatment outcome is probabilistic ) would be characterized by a steep dose response , and the number of patients required to demonstrate the effect of dose escalation would be substantially reduced ( by about 50 % ) .
	manualset3
163240	3	412151	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting `` stochastic fraction '' ( tumors for which treatment outcome is probabilistic ) would be characterized by a steep dose response , and the number of patients required to demonstrate the effect of dose escalation would be substantially reduced ( by about 50 % ) .
	manualset3
163241	4	412151	7	NULL	NULL	0	NULL	steep dose response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting `` stochastic fraction '' ( tumors for which treatment outcome is probabilistic ) would be characterized by a steep dose response , and the number of patients required to demonstrate the effect of dose escalation would be substantially reduced ( by about 50 % ) .
	manualset3
163242	5	412151	7	NULL	NULL	0	NULL	 number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting `` stochastic fraction '' ( tumors for which treatment outcome is probabilistic ) would be characterized by a steep dose response , and the number of patients required to demonstrate the effect of dose escalation would be substantially reduced ( by about 50 % ) .
	manualset3
163243	6	412151	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting `` stochastic fraction '' ( tumors for which treatment outcome is probabilistic ) would be characterized by a steep dose response , and the number of patients required to demonstrate the effect of dose escalation would be substantially reduced ( by about 50 % ) .
	manualset3
163244	7	412151	7	NULL	NULL	0	NULL	 effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting `` stochastic fraction '' ( tumors for which treatment outcome is probabilistic ) would be characterized by a steep dose response , and the number of patients required to demonstrate the effect of dose escalation would be substantially reduced ( by about 50 % ) .
	manualset3
163245	8	412151	7	NULL	NULL	0	NULL	 dose escalation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting `` stochastic fraction '' ( tumors for which treatment outcome is probabilistic ) would be characterized by a steep dose response , and the number of patients required to demonstrate the effect of dose escalation would be substantially reduced ( by about 50 % ) .
	manualset3
163246	9	412151	7	NULL	NULL	0	NULL	50 %	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting `` stochastic fraction '' ( tumors for which treatment outcome is probabilistic ) would be characterized by a steep dose response , and the number of patients required to demonstrate the effect of dose escalation would be substantially reduced ( by about 50 % ) .
	manualset3
163248	1	412152	7	NULL	NULL	0	NULL	aqueous layers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting aqueous layers can potentially be sewered ; whereas the organic layer can be recovered for potential reuse .
	manualset3
163249	2	412152	7	NULL	NULL	0	NULL	organic layer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting aqueous layers can potentially be sewered ; whereas the organic layer can be recovered for potential reuse .
	manualset3
169727	3	412152	7	NULL	NULL	0	NULL	potential reuse	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting aqueous layers can potentially be sewered ; whereas the organic layer can be recovered for potential reuse .
	manualset3
163251	1	412153	7	NULL	NULL	0	NULL	Absorbed doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Absorbed doses to QGP and Bon1 cells are up to 150 and 30 Gy , respectively .
	manualset3
163252	2	412153	7	NULL	NULL	0	NULL	QGP cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Absorbed doses to QGP and Bon1 cells are up to 150 and 30 Gy , respectively .
	manualset3
163253	3	412153	7	NULL	NULL	0	NULL	Bon1 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Absorbed doses to QGP and Bon1 cells are up to 150 and 30 Gy , respectively .
	manualset3
163254	4	412153	7	NULL	NULL	0	NULL	150 Gy	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Absorbed doses to QGP and Bon1 cells are up to 150 and 30 Gy , respectively .
	manualset3
163255	5	412153	7	NULL	NULL	0	NULL	30 Gy	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Absorbed doses to QGP and Bon1 cells are up to 150 and 30 Gy , respectively .
	manualset3
163256	1	412154	7	NULL	NULL	0	NULL	bimetallic Nd/Mg system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting bimetallic Nd/Mg system behaves as an efficient and highly stereospecific catalyst with the synthesis of trans-1 , 4 - polyisoprene with more than 98 % regularity .
	manualset3
163257	2	412154	7	NULL	NULL	0	NULL	stereospecific catalyst	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting bimetallic Nd/Mg system behaves as an efficient and highly stereospecific catalyst with the synthesis of trans-1 , 4 - polyisoprene with more than 98 % regularity .
	manualset3
163258	3	412154	7	NULL	NULL	0	NULL	synthesis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting bimetallic Nd/Mg system behaves as an efficient and highly stereospecific catalyst with the synthesis of trans-1 , 4 - polyisoprene with more than 98 % regularity .
	manualset3
163259	4	412154	7	NULL	NULL	0	NULL	trans-1 , 4 - polyisoprene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting bimetallic Nd/Mg system behaves as an efficient and highly stereospecific catalyst with the synthesis of trans-1 , 4 - polyisoprene with more than 98 % regularity .
	manualset3
163260	5	412154	7	NULL	NULL	0	NULL	98 %	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting bimetallic Nd/Mg system behaves as an efficient and highly stereospecific catalyst with the synthesis of trans-1 , 4 - polyisoprene with more than 98 % regularity .
	manualset3
169728	6	412154	7	NULL	NULL	0	NULL	regularity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting bimetallic Nd/Mg system behaves as an efficient and highly stereospecific catalyst with the synthesis of trans-1 , 4 - polyisoprene with more than 98 % regularity .
	manualset3
163262	1	412155	7	NULL	NULL	NULL	NULL	cell	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The resulting cell is metabolically dormant and as close to indestructible as any cell found on earth .
	manualset3
163263	2	412155	7	NULL	NULL	0	NULL	metabolically dormant	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting cell is metabolically dormant and as close to indestructible as any cell found on earth .
	manualset3
163265	3	412155	7	NULL	NULL	0	NULL	cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting cell is metabolically dormant and as close to indestructible as any cell found on earth .
	manualset3
163266	4	412155	7	NULL	NULL	0	NULL	earth 	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting cell is metabolically dormant and as close to indestructible as any cell found on earth .
	manualset3
163267	1	412156	7	NULL	NULL	0	NULL	dose-volume histograms	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting dose-volume histograms were compared with those obtained from conventional photon and electron treatment techniques in our clinic , which included IMRT , electron beam and mixed beams , most of them using fixed-thickness bolus .
	manualset3
163268	2	412156	7	NULL	NULL	0	NULL	conventional photon technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting dose-volume histograms were compared with those obtained from conventional photon and electron treatment techniques in our clinic , which included IMRT , electron beam and mixed beams , most of them using fixed-thickness bolus .
	manualset3
163269	3	412156	7	NULL	NULL	0	NULL	electron treatment techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting dose-volume histograms were compared with those obtained from conventional photon and electron treatment techniques in our clinic , which included IMRT , electron beam and mixed beams , most of them using fixed-thickness bolus .
	manualset3
163270	4	412156	7	NULL	NULL	0	NULL	clinic	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting dose-volume histograms were compared with those obtained from conventional photon and electron treatment techniques in our clinic , which included IMRT , electron beam and mixed beams , most of them using fixed-thickness bolus .
	manualset3
163271	5	412156	7	NULL	NULL	0	NULL	IMRT	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting dose-volume histograms were compared with those obtained from conventional photon and electron treatment techniques in our clinic , which included IMRT , electron beam and mixed beams , most of them using fixed-thickness bolus .
	manualset3
163272	6	412156	7	NULL	NULL	0	NULL	electron beam	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting dose-volume histograms were compared with those obtained from conventional photon and electron treatment techniques in our clinic , which included IMRT , electron beam and mixed beams , most of them using fixed-thickness bolus .
	manualset3
163273	7	412156	7	NULL	NULL	0	NULL	mixed beams	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting dose-volume histograms were compared with those obtained from conventional photon and electron treatment techniques in our clinic , which included IMRT , electron beam and mixed beams , most of them using fixed-thickness bolus .
	manualset3
163274	8	412156	7	NULL	NULL	0	NULL	fixed-thickness bolus 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting dose-volume histograms were compared with those obtained from conventional photon and electron treatment techniques in our clinic , which included IMRT , electron beam and mixed beams , most of them using fixed-thickness bolus .
	manualset3
163275	1	412157	7	NULL	NULL	NULL	NULL	 films 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The resulting films transport electrons efficiently from the electrode surface to the film/solution interface .
	manualset3
163276	2	412157	7	NULL	NULL	NULL	NULL	electrons	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The resulting films transport electrons efficiently from the electrode surface to the film/solution interface .
	manualset3
163277	3	412157	7	NULL	NULL	NULL	NULL	electrode surface 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The resulting films transport electrons efficiently from the electrode surface to the film/solution interface .
	manualset3
163278	4	412157	7	NULL	NULL	NULL	NULL	film/solution interface	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The resulting films transport electrons efficiently from the electrode surface to the film/solution interface .
	manualset3
163279	1	412158	7	NULL	NULL	0	NULL	mass spectra	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting mass spectra of these substances show a significant increase in signal/chemical noise when compared to normal fast atom bombardment ( FAB ) mass spectra .
	manualset3
163280	2	412158	7	NULL	NULL	0	NULL	substances	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting mass spectra of these substances show a significant increase in signal/chemical noise when compared to normal fast atom bombardment ( FAB ) mass spectra .
	manualset3
163281	3	412158	7	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting mass spectra of these substances show a significant increase in signal/chemical noise when compared to normal fast atom bombardment ( FAB ) mass spectra .
	manualset3
163282	4	412158	7	NULL	NULL	0	NULL	signal/chemical noise	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting mass spectra of these substances show a significant increase in signal/chemical noise when compared to normal fast atom bombardment ( FAB ) mass spectra .
	manualset3
163283	5	412158	7	NULL	NULL	0	NULL	normal fast atom bombardment ( FAB ) mass spectra	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting mass spectra of these substances show a significant increase in signal/chemical noise when compared to normal fast atom bombardment ( FAB ) mass spectra .
	manualset3
163284	1	412159	7	NULL	NULL	0	NULL	myoblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting myoblasts expressed Myf5 and MyoD and differentiated into myotubes that expressed myogenin and myosin heavy chain .
	manualset3
163285	2	412159	7	NULL	NULL	NULL	NULL	Myf5	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The resulting myoblasts expressed Myf5 and MyoD and differentiated into myotubes that expressed myogenin and myosin heavy chain .
	manualset3
163286	3	412159	7	NULL	NULL	NULL	NULL	MyoD	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The resulting myoblasts expressed Myf5 and MyoD and differentiated into myotubes that expressed myogenin and myosin heavy chain .
	manualset3
163287	4	412159	7	NULL	NULL	0	NULL	myotubes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting myoblasts expressed Myf5 and MyoD and differentiated into myotubes that expressed myogenin and myosin heavy chain .
	manualset3
163288	5	412159	7	NULL	NULL	0	NULL	myogenin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting myoblasts expressed Myf5 and MyoD and differentiated into myotubes that expressed myogenin and myosin heavy chain .
	manualset3
163289	6	412159	7	NULL	NULL	0	NULL	myosin heavy chain	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting myoblasts expressed Myf5 and MyoD and differentiated into myotubes that expressed myogenin and myosin heavy chain .
	manualset3
163290	1	412160	7	NULL	NULL	NULL	NULL	rapid reaction	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The resulting rapid reaction is thought to shift the reduction potentials for guanine and adenine to lower values than observed in RTILs where the scope for proton abstraction is not present .
	manualset3
163291	2	412160	7	NULL	NULL	0	NULL	reduction potentials 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting rapid reaction is thought to shift the reduction potentials for guanine and adenine to lower values than observed in RTILs where the scope for proton abstraction is not present .
	manualset3
163292	3	412160	7	NULL	NULL	0	NULL	guanine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting rapid reaction is thought to shift the reduction potentials for guanine and adenine to lower values than observed in RTILs where the scope for proton abstraction is not present .
	manualset3
163293	4	412160	7	NULL	NULL	0	NULL	adenine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting rapid reaction is thought to shift the reduction potentials for guanine and adenine to lower values than observed in RTILs where the scope for proton abstraction is not present .
	manualset3
163294	5	412160	7	NULL	NULL	0	NULL	lower values 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting rapid reaction is thought to shift the reduction potentials for guanine and adenine to lower values than observed in RTILs where the scope for proton abstraction is not present .
	manualset3
163295	6	412160	7	NULL	NULL	0	NULL	RTILs	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting rapid reaction is thought to shift the reduction potentials for guanine and adenine to lower values than observed in RTILs where the scope for proton abstraction is not present .
	manualset3
163296	7	412160	7	NULL	NULL	NULL	NULL	 scope	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The resulting rapid reaction is thought to shift the reduction potentials for guanine and adenine to lower values than observed in RTILs where the scope for proton abstraction is not present .
	manualset3
163297	8	412160	7	NULL	NULL	NULL	NULL	proton abstraction	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The resulting rapid reaction is thought to shift the reduction potentials for guanine and adenine to lower values than observed in RTILs where the scope for proton abstraction is not present .
	manualset3
163298	1	412161	7	NULL	NULL	0	NULL	sensor plasmid 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting sensor plasmid pTOO24 is capable of replicating in Gram-positive and Gram-negative bacteria .
	manualset3
163299	2	412161	7	NULL	NULL	0	NULL	 pTOO24 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting sensor plasmid pTOO24 is capable of replicating in Gram-positive and Gram-negative bacteria .
	manualset3
163300	3	412161	7	NULL	NULL	0	NULL	Gram-positive bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting sensor plasmid pTOO24 is capable of replicating in Gram-positive and Gram-negative bacteria .
	manualset3
163301	4	412161	7	NULL	NULL	0	NULL	Gram-negative bacteria 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting sensor plasmid pTOO24 is capable of replicating in Gram-positive and Gram-negative bacteria .
	manualset3
163302	1	412162	7	NULL	NULL	0	NULL	vectors	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting vectors were introduced into three cultured lines of murine cells -- C127 , NIH3T3 and MME -- either alone or in the presence of a plasmid that carries the aminoglycoside transferase gene of Tn5 .
	manualset3
163303	2	412162	7	NULL	NULL	0	NULL	three cultured lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting vectors were introduced into three cultured lines of murine cells -- C127 , NIH3T3 and MME -- either alone or in the presence of a plasmid that carries the aminoglycoside transferase gene of Tn5 .
	manualset3
163304	3	412162	7	NULL	NULL	0	NULL	murine cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting vectors were introduced into three cultured lines of murine cells -- C127 , NIH3T3 and MME -- either alone or in the presence of a plasmid that carries the aminoglycoside transferase gene of Tn5 .
	manualset3
163305	4	412162	7	NULL	NULL	0	NULL	C127	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting vectors were introduced into three cultured lines of murine cells -- C127 , NIH3T3 and MME -- either alone or in the presence of a plasmid that carries the aminoglycoside transferase gene of Tn5 .
	manualset3
163306	5	412162	7	NULL	NULL	0	NULL	 NIH3T3	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting vectors were introduced into three cultured lines of murine cells -- C127 , NIH3T3 and MME -- either alone or in the presence of a plasmid that carries the aminoglycoside transferase gene of Tn5 .
	manualset3
163307	6	412162	7	NULL	NULL	0	NULL	MME	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting vectors were introduced into three cultured lines of murine cells -- C127 , NIH3T3 and MME -- either alone or in the presence of a plasmid that carries the aminoglycoside transferase gene of Tn5 .
	manualset3
163308	7	412162	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting vectors were introduced into three cultured lines of murine cells -- C127 , NIH3T3 and MME -- either alone or in the presence of a plasmid that carries the aminoglycoside transferase gene of Tn5 .
	manualset3
163309	8	412162	7	NULL	NULL	0	NULL	plasmid	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting vectors were introduced into three cultured lines of murine cells -- C127 , NIH3T3 and MME -- either alone or in the presence of a plasmid that carries the aminoglycoside transferase gene of Tn5 .
	manualset3
163310	9	412162	7	NULL	NULL	0	NULL	aminoglycoside transferase gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting vectors were introduced into three cultured lines of murine cells -- C127 , NIH3T3 and MME -- either alone or in the presence of a plasmid that carries the aminoglycoside transferase gene of Tn5 .
	manualset3
163311	10	412162	7	NULL	NULL	0	NULL	Tn5	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting vectors were introduced into three cultured lines of murine cells -- C127 , NIH3T3 and MME -- either alone or in the presence of a plasmid that carries the aminoglycoside transferase gene of Tn5 .
	manualset3
163312	1	412163	7	NULL	NULL	0	NULL	Clinical variants	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical variants of acute glomerulonephritis in children ) .
	manualset3
163313	2	412163	7	NULL	NULL	0	NULL	acute glomerulonephritis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical variants of acute glomerulonephritis in children ) .
	manualset3
163314	3	412163	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical variants of acute glomerulonephritis in children ) .
	manualset3
163315	1	412164	7	NULL	NULL	0	NULL	Absorbent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Absorbent and impermeable dressings were applied over the tunnel exit , catheter Luer connection and bacterial filter .
	manualset3
163316	2	412164	7	NULL	NULL	NULL	NULL	impermeable dressings	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Absorbent and impermeable dressings were applied over the tunnel exit , catheter Luer connection and bacterial filter .
	manualset3
163317	3	412164	7	NULL	NULL	NULL	NULL	 tunnel exit	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Absorbent and impermeable dressings were applied over the tunnel exit , catheter Luer connection and bacterial filter .
	manualset3
163318	4	412164	7	NULL	NULL	NULL	NULL	catheter Luer connection	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Absorbent and impermeable dressings were applied over the tunnel exit , catheter Luer connection and bacterial filter .
	manualset3
163319	5	412164	7	NULL	NULL	NULL	NULL	bacterial filter	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Absorbent and impermeable dressings were applied over the tunnel exit , catheter Luer connection and bacterial filter .
	manualset3
163320	1	412165	7	NULL	NULL	NULL	NULL	result	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results , in agreement with those obtained with conditioned media , show that each leukemic case displays a different pattern of response to CSFs , and that optimal growth conditions must be individually assessed .
	manualset3
163321	2	412165	7	NULL	NULL	0	NULL	agreement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results , in agreement with those obtained with conditioned media , show that each leukemic case displays a different pattern of response to CSFs , and that optimal growth conditions must be individually assessed .
	manualset3
163322	3	412165	7	NULL	NULL	0	NULL	conditioned media	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The results , in agreement with those obtained with conditioned media , show that each leukemic case displays a different pattern of response to CSFs , and that optimal growth conditions must be individually assessed .
	manualset3
163323	4	412165	7	NULL	NULL	0	NULL	 leukemic case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results , in agreement with those obtained with conditioned media , show that each leukemic case displays a different pattern of response to CSFs , and that optimal growth conditions must be individually assessed .
	manualset3
163324	5	412165	7	NULL	NULL	0	NULL	different pattern	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results , in agreement with those obtained with conditioned media , show that each leukemic case displays a different pattern of response to CSFs , and that optimal growth conditions must be individually assessed .
	manualset3
163325	6	412165	7	NULL	NULL	0	NULL	 response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results , in agreement with those obtained with conditioned media , show that each leukemic case displays a different pattern of response to CSFs , and that optimal growth conditions must be individually assessed .
	manualset3
163326	7	412165	7	NULL	NULL	0	NULL	CSFs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results , in agreement with those obtained with conditioned media , show that each leukemic case displays a different pattern of response to CSFs , and that optimal growth conditions must be individually assessed .
	manualset3
163327	8	412165	7	NULL	NULL	0	NULL	optimal growth conditions 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The results , in agreement with those obtained with conditioned media , show that each leukemic case displays a different pattern of response to CSFs , and that optimal growth conditions must be individually assessed .
	manualset3
163328	1	412166	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results : show that , for both materials uranium is cleared rapidly from the lungs , much of it to the blood , show that the distribution of uranium amongst body tissues , and the fraction of the systemic content excreted in urine , is similar to that obtained after the administration of U ( VI ) bicarbonate , show that the transportability of uranium is much greater than in previously reported studies with other preparations of uranium tetrafluoride , suggest that lung radioactivity counting measurements would be of limited value for interpreting human exposures , indicate that for setting exposure limits these tetrafluorides should be considered moderately transportable compounds ( ICRP inhalation class W ) .
	manualset3
163329	2	412166	7	NULL	NULL	0	NULL	materials uranium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results : show that , for both materials uranium is cleared rapidly from the lungs , much of it to the blood , show that the distribution of uranium amongst body tissues , and the fraction of the systemic content excreted in urine , is similar to that obtained after the administration of U ( VI ) bicarbonate , show that the transportability of uranium is much greater than in previously reported studies with other preparations of uranium tetrafluoride , suggest that lung radioactivity counting measurements would be of limited value for interpreting human exposures , indicate that for setting exposure limits these tetrafluorides should be considered moderately transportable compounds ( ICRP inhalation class W ) .
	manualset3
163330	3	412166	7	NULL	NULL	0	NULL	 lungs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results : show that , for both materials uranium is cleared rapidly from the lungs , much of it to the blood , show that the distribution of uranium amongst body tissues , and the fraction of the systemic content excreted in urine , is similar to that obtained after the administration of U ( VI ) bicarbonate , show that the transportability of uranium is much greater than in previously reported studies with other preparations of uranium tetrafluoride , suggest that lung radioactivity counting measurements would be of limited value for interpreting human exposures , indicate that for setting exposure limits these tetrafluorides should be considered moderately transportable compounds ( ICRP inhalation class W ) .
	manualset3
163331	4	412166	7	NULL	NULL	0	NULL	 blood 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results : show that , for both materials uranium is cleared rapidly from the lungs , much of it to the blood , show that the distribution of uranium amongst body tissues , and the fraction of the systemic content excreted in urine , is similar to that obtained after the administration of U ( VI ) bicarbonate , show that the transportability of uranium is much greater than in previously reported studies with other preparations of uranium tetrafluoride , suggest that lung radioactivity counting measurements would be of limited value for interpreting human exposures , indicate that for setting exposure limits these tetrafluorides should be considered moderately transportable compounds ( ICRP inhalation class W ) .
	manualset3
163332	5	412166	7	NULL	NULL	0	NULL	distribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results : show that , for both materials uranium is cleared rapidly from the lungs , much of it to the blood , show that the distribution of uranium amongst body tissues , and the fraction of the systemic content excreted in urine , is similar to that obtained after the administration of U ( VI ) bicarbonate , show that the transportability of uranium is much greater than in previously reported studies with other preparations of uranium tetrafluoride , suggest that lung radioactivity counting measurements would be of limited value for interpreting human exposures , indicate that for setting exposure limits these tetrafluorides should be considered moderately transportable compounds ( ICRP inhalation class W ) .
	manualset3
163333	6	412166	7	NULL	NULL	0	NULL	uranium 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results : show that , for both materials uranium is cleared rapidly from the lungs , much of it to the blood , show that the distribution of uranium amongst body tissues , and the fraction of the systemic content excreted in urine , is similar to that obtained after the administration of U ( VI ) bicarbonate , show that the transportability of uranium is much greater than in previously reported studies with other preparations of uranium tetrafluoride , suggest that lung radioactivity counting measurements would be of limited value for interpreting human exposures , indicate that for setting exposure limits these tetrafluorides should be considered moderately transportable compounds ( ICRP inhalation class W ) .
	manualset3
163334	7	412166	7	NULL	NULL	0	NULL	body tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The results : show that , for both materials uranium is cleared rapidly from the lungs , much of it to the blood , show that the distribution of uranium amongst body tissues , and the fraction of the systemic content excreted in urine , is similar to that obtained after the administration of U ( VI ) bicarbonate , show that the transportability of uranium is much greater than in previously reported studies with other preparations of uranium tetrafluoride , suggest that lung radioactivity counting measurements would be of limited value for interpreting human exposures , indicate that for setting exposure limits these tetrafluorides should be considered moderately transportable compounds ( ICRP inhalation class W ) .
	manualset3
163335	8	412166	7	NULL	NULL	0	NULL	fraction 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results : show that , for both materials uranium is cleared rapidly from the lungs , much of it to the blood , show that the distribution of uranium amongst body tissues , and the fraction of the systemic content excreted in urine , is similar to that obtained after the administration of U ( VI ) bicarbonate , show that the transportability of uranium is much greater than in previously reported studies with other preparations of uranium tetrafluoride , suggest that lung radioactivity counting measurements would be of limited value for interpreting human exposures , indicate that for setting exposure limits these tetrafluorides should be considered moderately transportable compounds ( ICRP inhalation class W ) .
	manualset3
163336	9	412166	7	NULL	NULL	0	NULL	 systemic content	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results : show that , for both materials uranium is cleared rapidly from the lungs , much of it to the blood , show that the distribution of uranium amongst body tissues , and the fraction of the systemic content excreted in urine , is similar to that obtained after the administration of U ( VI ) bicarbonate , show that the transportability of uranium is much greater than in previously reported studies with other preparations of uranium tetrafluoride , suggest that lung radioactivity counting measurements would be of limited value for interpreting human exposures , indicate that for setting exposure limits these tetrafluorides should be considered moderately transportable compounds ( ICRP inhalation class W ) .
	manualset3
163337	10	412166	7	NULL	NULL	0	NULL	 urine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results : show that , for both materials uranium is cleared rapidly from the lungs , much of it to the blood , show that the distribution of uranium amongst body tissues , and the fraction of the systemic content excreted in urine , is similar to that obtained after the administration of U ( VI ) bicarbonate , show that the transportability of uranium is much greater than in previously reported studies with other preparations of uranium tetrafluoride , suggest that lung radioactivity counting measurements would be of limited value for interpreting human exposures , indicate that for setting exposure limits these tetrafluorides should be considered moderately transportable compounds ( ICRP inhalation class W ) .
	manualset3
163338	11	412166	7	NULL	NULL	0	NULL	administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results : show that , for both materials uranium is cleared rapidly from the lungs , much of it to the blood , show that the distribution of uranium amongst body tissues , and the fraction of the systemic content excreted in urine , is similar to that obtained after the administration of U ( VI ) bicarbonate , show that the transportability of uranium is much greater than in previously reported studies with other preparations of uranium tetrafluoride , suggest that lung radioactivity counting measurements would be of limited value for interpreting human exposures , indicate that for setting exposure limits these tetrafluorides should be considered moderately transportable compounds ( ICRP inhalation class W ) .
	manualset3
163339	12	412166	7	NULL	NULL	0	NULL	 U ( VI ) bicarbonate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results : show that , for both materials uranium is cleared rapidly from the lungs , much of it to the blood , show that the distribution of uranium amongst body tissues , and the fraction of the systemic content excreted in urine , is similar to that obtained after the administration of U ( VI ) bicarbonate , show that the transportability of uranium is much greater than in previously reported studies with other preparations of uranium tetrafluoride , suggest that lung radioactivity counting measurements would be of limited value for interpreting human exposures , indicate that for setting exposure limits these tetrafluorides should be considered moderately transportable compounds ( ICRP inhalation class W ) .
	manualset3
163340	13	412166	7	NULL	NULL	0	NULL	transportability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results : show that , for both materials uranium is cleared rapidly from the lungs , much of it to the blood , show that the distribution of uranium amongst body tissues , and the fraction of the systemic content excreted in urine , is similar to that obtained after the administration of U ( VI ) bicarbonate , show that the transportability of uranium is much greater than in previously reported studies with other preparations of uranium tetrafluoride , suggest that lung radioactivity counting measurements would be of limited value for interpreting human exposures , indicate that for setting exposure limits these tetrafluorides should be considered moderately transportable compounds ( ICRP inhalation class W ) .
	manualset3
163341	14	412166	7	NULL	NULL	0	NULL	uranium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results : show that , for both materials uranium is cleared rapidly from the lungs , much of it to the blood , show that the distribution of uranium amongst body tissues , and the fraction of the systemic content excreted in urine , is similar to that obtained after the administration of U ( VI ) bicarbonate , show that the transportability of uranium is much greater than in previously reported studies with other preparations of uranium tetrafluoride , suggest that lung radioactivity counting measurements would be of limited value for interpreting human exposures , indicate that for setting exposure limits these tetrafluorides should be considered moderately transportable compounds ( ICRP inhalation class W ) .
	manualset3
163342	15	412166	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results : show that , for both materials uranium is cleared rapidly from the lungs , much of it to the blood , show that the distribution of uranium amongst body tissues , and the fraction of the systemic content excreted in urine , is similar to that obtained after the administration of U ( VI ) bicarbonate , show that the transportability of uranium is much greater than in previously reported studies with other preparations of uranium tetrafluoride , suggest that lung radioactivity counting measurements would be of limited value for interpreting human exposures , indicate that for setting exposure limits these tetrafluorides should be considered moderately transportable compounds ( ICRP inhalation class W ) .
	manualset3
163343	16	412166	7	NULL	NULL	NULL	NULL	preparations	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results : show that , for both materials uranium is cleared rapidly from the lungs , much of it to the blood , show that the distribution of uranium amongst body tissues , and the fraction of the systemic content excreted in urine , is similar to that obtained after the administration of U ( VI ) bicarbonate , show that the transportability of uranium is much greater than in previously reported studies with other preparations of uranium tetrafluoride , suggest that lung radioactivity counting measurements would be of limited value for interpreting human exposures , indicate that for setting exposure limits these tetrafluorides should be considered moderately transportable compounds ( ICRP inhalation class W ) .
	manualset3
163344	17	412166	7	NULL	NULL	0	NULL	 uranium tetrafluoride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results : show that , for both materials uranium is cleared rapidly from the lungs , much of it to the blood , show that the distribution of uranium amongst body tissues , and the fraction of the systemic content excreted in urine , is similar to that obtained after the administration of U ( VI ) bicarbonate , show that the transportability of uranium is much greater than in previously reported studies with other preparations of uranium tetrafluoride , suggest that lung radioactivity counting measurements would be of limited value for interpreting human exposures , indicate that for setting exposure limits these tetrafluorides should be considered moderately transportable compounds ( ICRP inhalation class W ) .
	manualset3
163345	18	412166	7	NULL	NULL	NULL	NULL	lung radioactivity counting measurements	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results : show that , for both materials uranium is cleared rapidly from the lungs , much of it to the blood , show that the distribution of uranium amongst body tissues , and the fraction of the systemic content excreted in urine , is similar to that obtained after the administration of U ( VI ) bicarbonate , show that the transportability of uranium is much greater than in previously reported studies with other preparations of uranium tetrafluoride , suggest that lung radioactivity counting measurements would be of limited value for interpreting human exposures , indicate that for setting exposure limits these tetrafluorides should be considered moderately transportable compounds ( ICRP inhalation class W ) .
	manualset3
163346	19	412166	7	NULL	NULL	0	NULL	limited value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results : show that , for both materials uranium is cleared rapidly from the lungs , much of it to the blood , show that the distribution of uranium amongst body tissues , and the fraction of the systemic content excreted in urine , is similar to that obtained after the administration of U ( VI ) bicarbonate , show that the transportability of uranium is much greater than in previously reported studies with other preparations of uranium tetrafluoride , suggest that lung radioactivity counting measurements would be of limited value for interpreting human exposures , indicate that for setting exposure limits these tetrafluorides should be considered moderately transportable compounds ( ICRP inhalation class W ) .
	manualset3
163347	20	412166	7	NULL	NULL	NULL	NULL	human exposures	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results : show that , for both materials uranium is cleared rapidly from the lungs , much of it to the blood , show that the distribution of uranium amongst body tissues , and the fraction of the systemic content excreted in urine , is similar to that obtained after the administration of U ( VI ) bicarbonate , show that the transportability of uranium is much greater than in previously reported studies with other preparations of uranium tetrafluoride , suggest that lung radioactivity counting measurements would be of limited value for interpreting human exposures , indicate that for setting exposure limits these tetrafluorides should be considered moderately transportable compounds ( ICRP inhalation class W ) .
	manualset3
163348	21	412166	7	NULL	NULL	0	NULL	exposure limits	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results : show that , for both materials uranium is cleared rapidly from the lungs , much of it to the blood , show that the distribution of uranium amongst body tissues , and the fraction of the systemic content excreted in urine , is similar to that obtained after the administration of U ( VI ) bicarbonate , show that the transportability of uranium is much greater than in previously reported studies with other preparations of uranium tetrafluoride , suggest that lung radioactivity counting measurements would be of limited value for interpreting human exposures , indicate that for setting exposure limits these tetrafluorides should be considered moderately transportable compounds ( ICRP inhalation class W ) .
	manualset3
163349	22	412166	7	NULL	NULL	0	NULL	tetrafluorides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results : show that , for both materials uranium is cleared rapidly from the lungs , much of it to the blood , show that the distribution of uranium amongst body tissues , and the fraction of the systemic content excreted in urine , is similar to that obtained after the administration of U ( VI ) bicarbonate , show that the transportability of uranium is much greater than in previously reported studies with other preparations of uranium tetrafluoride , suggest that lung radioactivity counting measurements would be of limited value for interpreting human exposures , indicate that for setting exposure limits these tetrafluorides should be considered moderately transportable compounds ( ICRP inhalation class W ) .
	manualset3
163350	23	412166	7	NULL	NULL	0	NULL	transportable compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results : show that , for both materials uranium is cleared rapidly from the lungs , much of it to the blood , show that the distribution of uranium amongst body tissues , and the fraction of the systemic content excreted in urine , is similar to that obtained after the administration of U ( VI ) bicarbonate , show that the transportability of uranium is much greater than in previously reported studies with other preparations of uranium tetrafluoride , suggest that lung radioactivity counting measurements would be of limited value for interpreting human exposures , indicate that for setting exposure limits these tetrafluorides should be considered moderately transportable compounds ( ICRP inhalation class W ) .
	manualset3
163351	24	412166	7	NULL	NULL	0	NULL	ICRP inhalation class W	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results : show that , for both materials uranium is cleared rapidly from the lungs , much of it to the blood , show that the distribution of uranium amongst body tissues , and the fraction of the systemic content excreted in urine , is similar to that obtained after the administration of U ( VI ) bicarbonate , show that the transportability of uranium is much greater than in previously reported studies with other preparations of uranium tetrafluoride , suggest that lung radioactivity counting measurements would be of limited value for interpreting human exposures , indicate that for setting exposure limits these tetrafluorides should be considered moderately transportable compounds ( ICRP inhalation class W ) .
	manualset3
163352	1	412167	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results also indicated that parental smoking status was associated with cough and phlegm , and use of coal in the home was associated only with cough prevalence ( alpha = 0.05 ) .
	manualset3
163353	2	412167	7	NULL	NULL	0	NULL	parental smoking status 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results also indicated that parental smoking status was associated with cough and phlegm , and use of coal in the home was associated only with cough prevalence ( alpha = 0.05 ) .
	manualset3
163354	3	412167	7	NULL	NULL	0	NULL	cough	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results also indicated that parental smoking status was associated with cough and phlegm , and use of coal in the home was associated only with cough prevalence ( alpha = 0.05 ) .
	manualset3
163355	4	412167	7	NULL	NULL	0	NULL	phlegm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results also indicated that parental smoking status was associated with cough and phlegm , and use of coal in the home was associated only with cough prevalence ( alpha = 0.05 ) .
	manualset3
163356	5	412167	7	NULL	NULL	0	NULL	coal	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results also indicated that parental smoking status was associated with cough and phlegm , and use of coal in the home was associated only with cough prevalence ( alpha = 0.05 ) .
	manualset3
163357	6	412167	7	NULL	NULL	0	NULL	home	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The results also indicated that parental smoking status was associated with cough and phlegm , and use of coal in the home was associated only with cough prevalence ( alpha = 0.05 ) .
	manualset3
163358	7	412167	7	NULL	NULL	0	NULL	cough 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results also indicated that parental smoking status was associated with cough and phlegm , and use of coal in the home was associated only with cough prevalence ( alpha = 0.05 ) .
	manualset3
163359	8	412167	7	NULL	NULL	0	NULL	alpha = 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results also indicated that parental smoking status was associated with cough and phlegm , and use of coal in the home was associated only with cough prevalence ( alpha = 0.05 ) .
	manualset3
163360	1	412168	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results also suggest that this area contributes to the generation of the electrical vertex potential .
	manualset3
163361	2	412168	7	NULL	NULL	NULL	NULL	area 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results also suggest that this area contributes to the generation of the electrical vertex potential .
	manualset3
163362	3	412168	7	NULL	NULL	0	NULL	 generation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results also suggest that this area contributes to the generation of the electrical vertex potential .
	manualset3
163363	4	412168	7	NULL	NULL	0	NULL	electrical vertex potential 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results also suggest that this area contributes to the generation of the electrical vertex potential .
	manualset3
163364	1	412169	7	NULL	NULL	NULL	NULL	results 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results are as follows : The spontaneous activity ( frequency and amplitude ) of isolated strips is extremely variable among strips of the same bladder .
	manualset3
163365	2	412169	7	NULL	NULL	0	NULL	spontaneous activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are as follows : The spontaneous activity ( frequency and amplitude ) of isolated strips is extremely variable among strips of the same bladder .
	manualset3
163366	3	412169	7	NULL	NULL	0	NULL	frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are as follows : The spontaneous activity ( frequency and amplitude ) of isolated strips is extremely variable among strips of the same bladder .
	manualset3
163367	4	412169	7	NULL	NULL	0	NULL	amplitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are as follows : The spontaneous activity ( frequency and amplitude ) of isolated strips is extremely variable among strips of the same bladder .
	manualset3
163368	5	412169	7	NULL	NULL	0	NULL	isolated strips	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are as follows : The spontaneous activity ( frequency and amplitude ) of isolated strips is extremely variable among strips of the same bladder .
	manualset3
163369	6	412169	7	NULL	NULL	0	NULL	strips	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are as follows : The spontaneous activity ( frequency and amplitude ) of isolated strips is extremely variable among strips of the same bladder .
	manualset3
163370	7	412169	7	NULL	NULL	0	NULL	bladder	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are as follows : The spontaneous activity ( frequency and amplitude ) of isolated strips is extremely variable among strips of the same bladder .
	manualset3
163371	1	412170	7	NULL	NULL	NULL	NULL	results 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results are compared to those obtained with the fat cell system , and an attempt is made to assess the universality principle .
	manualset3
163372	2	412170	7	NULL	NULL	0	NULL	fat cell system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are compared to those obtained with the fat cell system , and an attempt is made to assess the universality principle .
	manualset3
163373	3	412170	7	NULL	NULL	0	NULL	attempt	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are compared to those obtained with the fat cell system , and an attempt is made to assess the universality principle .
	manualset3
163374	4	412170	7	NULL	NULL	NULL	NULL	universality principle	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results are compared to those obtained with the fat cell system , and an attempt is made to assess the universality principle .
	manualset3
163375	1	412171	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results are compatible with the classification of R56865 as an inhibitor of Na + and Ca2 + overload .
	manualset3
163376	2	412171	7	NULL	NULL	0	NULL	classification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are compatible with the classification of R56865 as an inhibitor of Na + and Ca2 + overload .
	manualset3
163377	3	412171	7	NULL	NULL	0	NULL	R56865	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are compatible with the classification of R56865 as an inhibitor of Na + and Ca2 + overload .
	manualset3
163378	4	412171	7	NULL	NULL	0	NULL	 inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are compatible with the classification of R56865 as an inhibitor of Na + and Ca2 + overload .
	manualset3
163379	5	412171	7	NULL	NULL	0	NULL	Na + 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are compatible with the classification of R56865 as an inhibitor of Na + and Ca2 + overload .
	manualset3
163380	6	412171	7	NULL	NULL	0	NULL	Ca2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are compatible with the classification of R56865 as an inhibitor of Na + and Ca2 + overload .
	manualset3
163381	7	412171	7	NULL	NULL	0	NULL	overload 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are compatible with the classification of R56865 as an inhibitor of Na + and Ca2 + overload .
	manualset3
163382	1	412172	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are consistent with the hypothesis that VSCT neurones signal information on interneuronal transmission to motoneurones .
	manualset3
163383	2	412172	7	NULL	NULL	0	NULL	hypothesis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are consistent with the hypothesis that VSCT neurones signal information on interneuronal transmission to motoneurones .
	manualset3
163384	3	412172	7	NULL	NULL	0	NULL	VSCT neurones signal information	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are consistent with the hypothesis that VSCT neurones signal information on interneuronal transmission to motoneurones .
	manualset3
163385	4	412172	7	NULL	NULL	0	NULL	 interneuronal transmission	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are consistent with the hypothesis that VSCT neurones signal information on interneuronal transmission to motoneurones .
	manualset3
163386	5	412172	7	NULL	NULL	0	NULL	motoneurones	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are consistent with the hypothesis that VSCT neurones signal information on interneuronal transmission to motoneurones .
	manualset3
163387	1	412173	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results are consistent with the hypothesis that the PM cells release MM-like peptides just prior to each ecdysis .
	manualset3
163388	2	412173	7	NULL	NULL	0	NULL	hypothesis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are consistent with the hypothesis that the PM cells release MM-like peptides just prior to each ecdysis .
	manualset3
163389	3	412173	7	NULL	NULL	0	NULL	PM cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are consistent with the hypothesis that the PM cells release MM-like peptides just prior to each ecdysis .
	manualset3
163390	4	412173	7	NULL	NULL	0	NULL	MM-like peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are consistent with the hypothesis that the PM cells release MM-like peptides just prior to each ecdysis .
	manualset3
163391	5	412173	7	NULL	NULL	0	NULL	ecdysis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are consistent with the hypothesis that the PM cells release MM-like peptides just prior to each ecdysis .
	manualset3
163392	1	412174	7	NULL	NULL	0	NULL	Absorption 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Absorption of hyaluronan applied to the surface of intact skin .
	manualset3
163393	2	412174	7	NULL	NULL	0	NULL	hyaluronan	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Absorption of hyaluronan applied to the surface of intact skin .
	manualset3
163394	3	412174	7	NULL	NULL	0	NULL	surface 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Absorption of hyaluronan applied to the surface of intact skin .
	manualset3
163395	4	412174	7	NULL	NULL	0	NULL	 intact skin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Absorption of hyaluronan applied to the surface of intact skin .
	manualset3
163397	1	412175	7	NULL	NULL	NULL	NULL	results 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results are consistent with thyroid peroxidase - and lactoperoxidase-catalyzed oxidation of resorcinol derivatives to reactive radical species that covalently bind to amino acid residues unique to these two enzymes .
	manualset3
163398	2	412175	7	NULL	NULL	NULL	NULL	thyroid peroxidase - catalyzed oxidation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results are consistent with thyroid peroxidase - and lactoperoxidase-catalyzed oxidation of resorcinol derivatives to reactive radical species that covalently bind to amino acid residues unique to these two enzymes .
	manualset3
163399	3	412175	7	NULL	NULL	NULL	NULL	lactoperoxidase-catalyzed oxidation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results are consistent with thyroid peroxidase - and lactoperoxidase-catalyzed oxidation of resorcinol derivatives to reactive radical species that covalently bind to amino acid residues unique to these two enzymes .
	manualset3
163401	5	412175	7	NULL	NULL	0	NULL	resorcinol derivatives 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are consistent with thyroid peroxidase - and lactoperoxidase-catalyzed oxidation of resorcinol derivatives to reactive radical species that covalently bind to amino acid residues unique to these two enzymes .
	manualset3
163402	6	412175	7	NULL	NULL	0	NULL	reactive radical species	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are consistent with thyroid peroxidase - and lactoperoxidase-catalyzed oxidation of resorcinol derivatives to reactive radical species that covalently bind to amino acid residues unique to these two enzymes .
	manualset3
163403	7	412175	7	NULL	NULL	0	NULL	amino acid residues 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are consistent with thyroid peroxidase - and lactoperoxidase-catalyzed oxidation of resorcinol derivatives to reactive radical species that covalently bind to amino acid residues unique to these two enzymes .
	manualset3
163404	8	412175	7	NULL	NULL	NULL	NULL	two 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results are consistent with thyroid peroxidase - and lactoperoxidase-catalyzed oxidation of resorcinol derivatives to reactive radical species that covalently bind to amino acid residues unique to these two enzymes .
	manualset3
164582	9	412175	7	NULL	NULL	0	NULL	enzymes	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are consistent with thyroid peroxidase - and lactoperoxidase-catalyzed oxidation of resorcinol derivatives to reactive radical species that covalently bind to amino acid residues unique to these two enzymes .
	manualset3
163405	1	412176	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results are discussed in connection with programmed cell death , mitochondrial activity , and heartwood formation .
	manualset3
163406	2	412176	7	NULL	NULL	0	NULL	connection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are discussed in connection with programmed cell death , mitochondrial activity , and heartwood formation .
	manualset3
163407	3	412176	7	NULL	NULL	0	NULL	 programmed cell death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are discussed in connection with programmed cell death , mitochondrial activity , and heartwood formation .
	manualset3
163408	4	412176	7	NULL	NULL	NULL	NULL	mitochondrial activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results are discussed in connection with programmed cell death , mitochondrial activity , and heartwood formation .
	manualset3
163409	5	412176	7	NULL	NULL	0	NULL	heartwood formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are discussed in connection with programmed cell death , mitochondrial activity , and heartwood formation .
	manualset3
163410	1	412177	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results are discussed in relation to the use of tannic acid as a protein fixative in electron microscopy .
	manualset3
163411	2	412177	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are discussed in relation to the use of tannic acid as a protein fixative in electron microscopy .
	manualset3
163413	4	412177	7	NULL	NULL	0	NULL	 tannic acid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are discussed in relation to the use of tannic acid as a protein fixative in electron microscopy .
	manualset3
163414	5	412177	7	NULL	NULL	0	NULL	protein fixative	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are discussed in relation to the use of tannic acid as a protein fixative in electron microscopy .
	manualset3
163415	6	412177	7	NULL	NULL	0	NULL	electron microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are discussed in relation to the use of tannic acid as a protein fixative in electron microscopy .
	manualset3
169729	7	412177	7	NULL	NULL	0	NULL	use	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are discussed in relation to the use of tannic acid as a protein fixative in electron microscopy .
	manualset3
163416	1	412178	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results are discussed in terms of the relationship between 19S and 7S globulin-producing cells .
	manualset3
163417	2	412178	7	NULL	NULL	0	NULL	 relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are discussed in terms of the relationship between 19S and 7S globulin-producing cells .
	manualset3
163418	3	412178	7	NULL	NULL	0	NULL	19S  globulin-producing cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are discussed in terms of the relationship between 19S and 7S globulin-producing cells .
	manualset3
163419	4	412178	7	NULL	NULL	0	NULL	7S globulin-producing cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are discussed in terms of the relationship between 19S and 7S globulin-producing cells .
	manualset3
163420	1	412179	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results are interesting in view of the complex evolution of the annexin gene family , and also point to the potential usefulness of echinoderm eggs as a model system in which to study annexin function .
	manualset3
163421	2	412179	7	NULL	NULL	NULL	NULL	complex evolution	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results are interesting in view of the complex evolution of the annexin gene family , and also point to the potential usefulness of echinoderm eggs as a model system in which to study annexin function .
	manualset3
163422	3	412179	7	NULL	NULL	0	NULL	annexin gene family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are interesting in view of the complex evolution of the annexin gene family , and also point to the potential usefulness of echinoderm eggs as a model system in which to study annexin function .
	manualset3
163423	4	412179	7	NULL	NULL	NULL	NULL	usefulness	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results are interesting in view of the complex evolution of the annexin gene family , and also point to the potential usefulness of echinoderm eggs as a model system in which to study annexin function .
	manualset3
163424	5	412179	7	NULL	NULL	0	NULL	echinoderm eggs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are interesting in view of the complex evolution of the annexin gene family , and also point to the potential usefulness of echinoderm eggs as a model system in which to study annexin function .
	manualset3
163425	6	412179	7	NULL	NULL	0	NULL	model system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are interesting in view of the complex evolution of the annexin gene family , and also point to the potential usefulness of echinoderm eggs as a model system in which to study annexin function .
	manualset3
163426	7	412179	7	NULL	NULL	NULL	NULL	annexin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results are interesting in view of the complex evolution of the annexin gene family , and also point to the potential usefulness of echinoderm eggs as a model system in which to study annexin function .
	manualset3
164156	8	412179	7	NULL	NULL	0	NULL	function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are interesting in view of the complex evolution of the annexin gene family , and also point to the potential usefulness of echinoderm eggs as a model system in which to study annexin function .
	manualset3
163427	1	412180	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results are presented as statistical models that could assist decisions about dispersant use in the vicinity of fish spawning habitats .
	manualset3
163428	2	412180	7	NULL	NULL	0	NULL	statistical models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are presented as statistical models that could assist decisions about dispersant use in the vicinity of fish spawning habitats .
	manualset3
163429	3	412180	7	NULL	NULL	0	NULL	 decisions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are presented as statistical models that could assist decisions about dispersant use in the vicinity of fish spawning habitats .
	manualset3
163430	4	412180	7	NULL	NULL	0	NULL	dispersant	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are presented as statistical models that could assist decisions about dispersant use in the vicinity of fish spawning habitats .
	manualset3
163431	5	412180	7	NULL	NULL	0	NULL	vicinity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are presented as statistical models that could assist decisions about dispersant use in the vicinity of fish spawning habitats .
	manualset3
163432	6	412180	7	NULL	NULL	0	NULL	 fish spawning habitats	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are presented as statistical models that could assist decisions about dispersant use in the vicinity of fish spawning habitats .
	manualset3
163433	1	412181	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results are similar for both callus cells and regenerants and provide further evidence that translocations take place in tissue culture .
	manualset3
163434	2	412181	7	NULL	NULL	0	NULL	callus cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are similar for both callus cells and regenerants and provide further evidence that translocations take place in tissue culture .
	manualset3
163435	3	412181	7	NULL	NULL	0	NULL	 regenerants	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are similar for both callus cells and regenerants and provide further evidence that translocations take place in tissue culture .
	manualset3
163436	4	412181	7	NULL	NULL	0	NULL	evidence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are similar for both callus cells and regenerants and provide further evidence that translocations take place in tissue culture .
	manualset3
163437	5	412181	7	NULL	NULL	NULL	NULL	translocations	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results are similar for both callus cells and regenerants and provide further evidence that translocations take place in tissue culture .
	manualset3
163438	6	412181	7	NULL	NULL	0	NULL	tissue culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The results are similar for both callus cells and regenerants and provide further evidence that translocations take place in tissue culture .
	manualset3
163439	1	412182	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results complement neurophysiological evidence and are consistent with the hypothesis that OBEs represent a breakdown in the normal binding of bodily-self sensations and suggest that out-of-body feelings ( OBFs ) are consequences of anomalous V-M experiences and precursors to a particular form of autoscopic experience , out-of-body autoscopy ( OBA ) .
	manualset3
163440	2	412182	7	NULL	NULL	NULL	NULL	neurophysiological evidence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results complement neurophysiological evidence and are consistent with the hypothesis that OBEs represent a breakdown in the normal binding of bodily-self sensations and suggest that out-of-body feelings ( OBFs ) are consequences of anomalous V-M experiences and precursors to a particular form of autoscopic experience , out-of-body autoscopy ( OBA ) .
	manualset3
163441	3	412182	7	NULL	NULL	0	NULL	hypothesis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results complement neurophysiological evidence and are consistent with the hypothesis that OBEs represent a breakdown in the normal binding of bodily-self sensations and suggest that out-of-body feelings ( OBFs ) are consequences of anomalous V-M experiences and precursors to a particular form of autoscopic experience , out-of-body autoscopy ( OBA ) .
	manualset3
163442	4	412182	7	NULL	NULL	NULL	NULL	OBEs	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results complement neurophysiological evidence and are consistent with the hypothesis that OBEs represent a breakdown in the normal binding of bodily-self sensations and suggest that out-of-body feelings ( OBFs ) are consequences of anomalous V-M experiences and precursors to a particular form of autoscopic experience , out-of-body autoscopy ( OBA ) .
	manualset3
163443	5	412182	7	NULL	NULL	NULL	NULL	breakdown	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results complement neurophysiological evidence and are consistent with the hypothesis that OBEs represent a breakdown in the normal binding of bodily-self sensations and suggest that out-of-body feelings ( OBFs ) are consequences of anomalous V-M experiences and precursors to a particular form of autoscopic experience , out-of-body autoscopy ( OBA ) .
	manualset3
163444	6	412182	7	NULL	NULL	NULL	NULL	normal binding	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results complement neurophysiological evidence and are consistent with the hypothesis that OBEs represent a breakdown in the normal binding of bodily-self sensations and suggest that out-of-body feelings ( OBFs ) are consequences of anomalous V-M experiences and precursors to a particular form of autoscopic experience , out-of-body autoscopy ( OBA ) .
	manualset3
163445	7	412182	7	NULL	NULL	NULL	NULL	bodily-self sensations	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results complement neurophysiological evidence and are consistent with the hypothesis that OBEs represent a breakdown in the normal binding of bodily-self sensations and suggest that out-of-body feelings ( OBFs ) are consequences of anomalous V-M experiences and precursors to a particular form of autoscopic experience , out-of-body autoscopy ( OBA ) .
	manualset3
163446	8	412182	7	NULL	NULL	NULL	NULL	out-of-body feelings ( OBFs )	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results complement neurophysiological evidence and are consistent with the hypothesis that OBEs represent a breakdown in the normal binding of bodily-self sensations and suggest that out-of-body feelings ( OBFs ) are consequences of anomalous V-M experiences and precursors to a particular form of autoscopic experience , out-of-body autoscopy ( OBA ) .
	manualset3
163447	9	412182	7	NULL	NULL	NULL	NULL	V-M experiences	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results complement neurophysiological evidence and are consistent with the hypothesis that OBEs represent a breakdown in the normal binding of bodily-self sensations and suggest that out-of-body feelings ( OBFs ) are consequences of anomalous V-M experiences and precursors to a particular form of autoscopic experience , out-of-body autoscopy ( OBA ) .
	manualset3
163448	10	412182	7	NULL	NULL	NULL	NULL	precursors	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results complement neurophysiological evidence and are consistent with the hypothesis that OBEs represent a breakdown in the normal binding of bodily-self sensations and suggest that out-of-body feelings ( OBFs ) are consequences of anomalous V-M experiences and precursors to a particular form of autoscopic experience , out-of-body autoscopy ( OBA ) .
	manualset3
163449	11	412182	7	NULL	NULL	0	NULL	 autoscopic experience	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results complement neurophysiological evidence and are consistent with the hypothesis that OBEs represent a breakdown in the normal binding of bodily-self sensations and suggest that out-of-body feelings ( OBFs ) are consequences of anomalous V-M experiences and precursors to a particular form of autoscopic experience , out-of-body autoscopy ( OBA ) .
	manualset3
163450	12	412182	7	NULL	NULL	NULL	NULL	out-of-body autoscopy ( OBA )	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results complement neurophysiological evidence and are consistent with the hypothesis that OBEs represent a breakdown in the normal binding of bodily-self sensations and suggest that out-of-body feelings ( OBFs ) are consequences of anomalous V-M experiences and precursors to a particular form of autoscopic experience , out-of-body autoscopy ( OBA ) .
	manualset3
163451	1	412183	7	NULL	NULL	0	NULL	Absorption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Absorption of monosaccharides in the postnatal period : age-specific changes .
	manualset3
163452	2	412183	7	NULL	NULL	0	NULL	monosaccharides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Absorption of monosaccharides in the postnatal period : age-specific changes .
	manualset3
163453	3	412183	7	NULL	NULL	0	NULL	postnatal period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Absorption of monosaccharides in the postnatal period : age-specific changes .
	manualset3
163454	4	412183	7	NULL	NULL	0	NULL	age-specific changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Absorption of monosaccharides in the postnatal period : age-specific changes .
	manualset3
163455	1	412184	7	NULL	NULL	0	NULL	results	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results confirm a marked asymmetry in the positional distribution of the fatty acids in all triacylglycerol samples , with the palmitic acid predominantly in the sn-1-position , the unsaturated acids about equally divided between the sn-2 - and sn-3-positions , and the stearic acid divided about equally between the sn-1 - and sn-3-positions .
	manualset3
163456	2	412184	7	NULL	NULL	0	NULL	marked asymmetry	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results confirm a marked asymmetry in the positional distribution of the fatty acids in all triacylglycerol samples , with the palmitic acid predominantly in the sn-1-position , the unsaturated acids about equally divided between the sn-2 - and sn-3-positions , and the stearic acid divided about equally between the sn-1 - and sn-3-positions .
	manualset3
163457	3	412184	7	NULL	NULL	0	NULL	positional distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results confirm a marked asymmetry in the positional distribution of the fatty acids in all triacylglycerol samples , with the palmitic acid predominantly in the sn-1-position , the unsaturated acids about equally divided between the sn-2 - and sn-3-positions , and the stearic acid divided about equally between the sn-1 - and sn-3-positions .
	manualset3
163458	4	412184	7	NULL	NULL	0	NULL	fatty acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results confirm a marked asymmetry in the positional distribution of the fatty acids in all triacylglycerol samples , with the palmitic acid predominantly in the sn-1-position , the unsaturated acids about equally divided between the sn-2 - and sn-3-positions , and the stearic acid divided about equally between the sn-1 - and sn-3-positions .
	manualset3
163459	5	412184	7	NULL	NULL	0	NULL	triacylglycerol samples	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results confirm a marked asymmetry in the positional distribution of the fatty acids in all triacylglycerol samples , with the palmitic acid predominantly in the sn-1-position , the unsaturated acids about equally divided between the sn-2 - and sn-3-positions , and the stearic acid divided about equally between the sn-1 - and sn-3-positions .
	manualset3
163460	6	412184	7	NULL	NULL	0	NULL	palmitic acid	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results confirm a marked asymmetry in the positional distribution of the fatty acids in all triacylglycerol samples , with the palmitic acid predominantly in the sn-1-position , the unsaturated acids about equally divided between the sn-2 - and sn-3-positions , and the stearic acid divided about equally between the sn-1 - and sn-3-positions .
	manualset3
163461	7	412184	7	NULL	NULL	0	NULL	sn-1-position	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results confirm a marked asymmetry in the positional distribution of the fatty acids in all triacylglycerol samples , with the palmitic acid predominantly in the sn-1-position , the unsaturated acids about equally divided between the sn-2 - and sn-3-positions , and the stearic acid divided about equally between the sn-1 - and sn-3-positions .
	manualset3
163462	8	412184	7	NULL	NULL	0	NULL	unsaturated acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results confirm a marked asymmetry in the positional distribution of the fatty acids in all triacylglycerol samples , with the palmitic acid predominantly in the sn-1-position , the unsaturated acids about equally divided between the sn-2 - and sn-3-positions , and the stearic acid divided about equally between the sn-1 - and sn-3-positions .
	manualset3
163463	9	412184	7	NULL	NULL	0	NULL	sn-2 -positions	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results confirm a marked asymmetry in the positional distribution of the fatty acids in all triacylglycerol samples , with the palmitic acid predominantly in the sn-1-position , the unsaturated acids about equally divided between the sn-2 - and sn-3-positions , and the stearic acid divided about equally between the sn-1 - and sn-3-positions .
	manualset3
163464	10	412184	7	NULL	NULL	0	NULL	sn-3-positions	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results confirm a marked asymmetry in the positional distribution of the fatty acids in all triacylglycerol samples , with the palmitic acid predominantly in the sn-1-position , the unsaturated acids about equally divided between the sn-2 - and sn-3-positions , and the stearic acid divided about equally between the sn-1 - and sn-3-positions .
	manualset3
163465	11	412184	7	NULL	NULL	0	NULL	stearic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results confirm a marked asymmetry in the positional distribution of the fatty acids in all triacylglycerol samples , with the palmitic acid predominantly in the sn-1-position , the unsaturated acids about equally divided between the sn-2 - and sn-3-positions , and the stearic acid divided about equally between the sn-1 - and sn-3-positions .
	manualset3
163466	12	412184	7	NULL	NULL	0	NULL	sn-1 -position	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results confirm a marked asymmetry in the positional distribution of the fatty acids in all triacylglycerol samples , with the palmitic acid predominantly in the sn-1-position , the unsaturated acids about equally divided between the sn-2 - and sn-3-positions , and the stearic acid divided about equally between the sn-1 - and sn-3-positions .
	manualset3
163467	13	412184	7	NULL	NULL	0	NULL	sn-3-positions 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results confirm a marked asymmetry in the positional distribution of the fatty acids in all triacylglycerol samples , with the palmitic acid predominantly in the sn-1-position , the unsaturated acids about equally divided between the sn-2 - and sn-3-positions , and the stearic acid divided about equally between the sn-1 - and sn-3-positions .
	manualset3
163468	1	412185	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results confirm gender differences in substance use and demonstrate that there are different patterns of substance use between ethnic groups .
	manualset3
163469	2	412185	7	NULL	NULL	NULL	NULL	gender differences 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results confirm gender differences in substance use and demonstrate that there are different patterns of substance use between ethnic groups .
	manualset3
163470	3	412185	7	NULL	NULL	NULL	NULL	substance use	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results confirm gender differences in substance use and demonstrate that there are different patterns of substance use between ethnic groups .
	manualset3
163471	4	412185	7	NULL	NULL	NULL	NULL	 substance use	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results confirm gender differences in substance use and demonstrate that there are different patterns of substance use between ethnic groups .
	manualset3
163472	5	412185	7	NULL	NULL	0	NULL	ethnic groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results confirm gender differences in substance use and demonstrate that there are different patterns of substance use between ethnic groups .
	manualset3
164856	6	412185	7	NULL	NULL	0	NULL	 different patterns	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results confirm gender differences in substance use and demonstrate that there are different patterns of substance use between ethnic groups .
	manualset3
163473	1	412186	7	NULL	NULL	NULL	NULL	 results 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results confirmed the need for improved professional training , adequacy of health services , and effective public policy to provide qualified health care for the elderly population .
	manualset3
163474	2	412186	7	NULL	NULL	0	NULL	 professional training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results confirmed the need for improved professional training , adequacy of health services , and effective public policy to provide qualified health care for the elderly population .
	manualset3
163475	3	412186	7	NULL	NULL	0	NULL	health services	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The results confirmed the need for improved professional training , adequacy of health services , and effective public policy to provide qualified health care for the elderly population .
	manualset3
163476	4	412186	7	NULL	NULL	0	NULL	 public policy	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The results confirmed the need for improved professional training , adequacy of health services , and effective public policy to provide qualified health care for the elderly population .
	manualset3
163477	5	412186	7	NULL	NULL	0	NULL	health care	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The results confirmed the need for improved professional training , adequacy of health services , and effective public policy to provide qualified health care for the elderly population .
	manualset3
163478	6	412186	7	NULL	NULL	0	NULL	elderly population 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results confirmed the need for improved professional training , adequacy of health services , and effective public policy to provide qualified health care for the elderly population .
	manualset3
163479	1	412187	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results demonstrate that cysteamine can stimulate immunoreactive gastrin secretion without any change in somatostatinlike immunoreactivity release .
	manualset3
163480	2	412187	7	NULL	NULL	0	NULL	cysteamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results demonstrate that cysteamine can stimulate immunoreactive gastrin secretion without any change in somatostatinlike immunoreactivity release .
	manualset3
163481	3	412187	7	NULL	NULL	NULL	NULL	gastrin secretion 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results demonstrate that cysteamine can stimulate immunoreactive gastrin secretion without any change in somatostatinlike immunoreactivity release .
	manualset3
163482	4	412187	7	NULL	NULL	0	NULL	somatostatinlike immunoreactivity release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results demonstrate that cysteamine can stimulate immunoreactive gastrin secretion without any change in somatostatinlike immunoreactivity release .
	manualset3
163483	1	412188	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results demonstrate that the ECL intensity depends largely on the length of the saturated carbon chain linkage : the longer is the carbon chain , the higher is the ECL intensity .
	manualset3
163484	2	412188	7	NULL	NULL	0	NULL	ECL intensity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results demonstrate that the ECL intensity depends largely on the length of the saturated carbon chain linkage : the longer is the carbon chain , the higher is the ECL intensity .
	manualset3
163485	3	412188	7	NULL	NULL	0	NULL	length 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results demonstrate that the ECL intensity depends largely on the length of the saturated carbon chain linkage : the longer is the carbon chain , the higher is the ECL intensity .
	manualset3
163486	4	412188	7	NULL	NULL	NULL	NULL	saturated carbon chain linkage	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results demonstrate that the ECL intensity depends largely on the length of the saturated carbon chain linkage : the longer is the carbon chain , the higher is the ECL intensity .
	manualset3
163487	5	412188	7	NULL	NULL	0	NULL	carbon chain 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results demonstrate that the ECL intensity depends largely on the length of the saturated carbon chain linkage : the longer is the carbon chain , the higher is the ECL intensity .
	manualset3
163488	6	412188	7	NULL	NULL	0	NULL	ECL intensity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results demonstrate that the ECL intensity depends largely on the length of the saturated carbon chain linkage : the longer is the carbon chain , the higher is the ECL intensity .
	manualset3
163489	1	412189	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results demonstrate the sensitivity of nucleolar proliferation in SON to environmental changes ranging from osmotic to neurogenic stress .
	manualset3
163490	2	412189	7	NULL	NULL	0	NULL	 sensitivity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results demonstrate the sensitivity of nucleolar proliferation in SON to environmental changes ranging from osmotic to neurogenic stress .
	manualset3
163491	3	412189	7	NULL	NULL	0	NULL	nucleolar proliferation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results demonstrate the sensitivity of nucleolar proliferation in SON to environmental changes ranging from osmotic to neurogenic stress .
	manualset3
163492	4	412189	7	NULL	NULL	0	NULL	SON	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The results demonstrate the sensitivity of nucleolar proliferation in SON to environmental changes ranging from osmotic to neurogenic stress .
	manualset3
163493	5	412189	7	NULL	NULL	NULL	NULL	osmotic stress	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results demonstrate the sensitivity of nucleolar proliferation in SON to environmental changes ranging from osmotic to neurogenic stress .
	manualset3
163494	6	412189	7	NULL	NULL	NULL	NULL	neurogenic stress	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results demonstrate the sensitivity of nucleolar proliferation in SON to environmental changes ranging from osmotic to neurogenic stress .
	manualset3
163495	1	412190	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results demonstrated that bio-printing of VEGF-containing fibrin gel supported sustained release of the GF in the collagen scaffold .
	manualset3
163496	2	412190	7	NULL	NULL	0	NULL	bio-printing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results demonstrated that bio-printing of VEGF-containing fibrin gel supported sustained release of the GF in the collagen scaffold .
	manualset3
163497	3	412190	7	NULL	NULL	0	NULL	VEGF-containing fibrin gel	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results demonstrated that bio-printing of VEGF-containing fibrin gel supported sustained release of the GF in the collagen scaffold .
	manualset3
163498	4	412190	7	NULL	NULL	0	NULL	release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results demonstrated that bio-printing of VEGF-containing fibrin gel supported sustained release of the GF in the collagen scaffold .
	manualset3
163499	5	412190	7	NULL	NULL	0	NULL	 GF 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results demonstrated that bio-printing of VEGF-containing fibrin gel supported sustained release of the GF in the collagen scaffold .
	manualset3
163500	6	412190	7	NULL	NULL	0	NULL	collagen scaffold 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results demonstrated that bio-printing of VEGF-containing fibrin gel supported sustained release of the GF in the collagen scaffold .
	manualset3
163501	1	412191	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results demonstrated that restriction fragment length of the DNA could be used as a means to distinguish isomorphic species of the Anopheles dirus .
	manualset3
163502	2	412191	7	NULL	NULL	0	NULL	 restriction fragment length 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results demonstrated that restriction fragment length of the DNA could be used as a means to distinguish isomorphic species of the Anopheles dirus .
	manualset3
163503	3	412191	7	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The results demonstrated that restriction fragment length of the DNA could be used as a means to distinguish isomorphic species of the Anopheles dirus .
	manualset3
163504	4	412191	7	NULL	NULL	0	NULL	isomorphic species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results demonstrated that restriction fragment length of the DNA could be used as a means to distinguish isomorphic species of the Anopheles dirus .
	manualset3
163505	5	412191	7	NULL	NULL	0	NULL	 Anopheles dirus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results demonstrated that restriction fragment length of the DNA could be used as a means to distinguish isomorphic species of the Anopheles dirus .
	manualset3
163506	6	412191	7	NULL	NULL	0	NULL	means	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results demonstrated that restriction fragment length of the DNA could be used as a means to distinguish isomorphic species of the Anopheles dirus .
	manualset3
163507	1	412192	7	NULL	NULL	NULL	NULL	 results 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results followed suit : The test-similar condition produced significantly elevated false alarms , relative to both the study-similar and the no-load conditions .
	manualset3
163508	2	412192	7	NULL	NULL	0	NULL	test-similar condition	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The results followed suit : The test-similar condition produced significantly elevated false alarms , relative to both the study-similar and the no-load conditions .
	manualset3
163509	3	412192	7	NULL	NULL	0	NULL	elevated false alarms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results followed suit : The test-similar condition produced significantly elevated false alarms , relative to both the study-similar and the no-load conditions .
	manualset3
163510	4	412192	7	NULL	NULL	0	NULL	study-similar condition 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The results followed suit : The test-similar condition produced significantly elevated false alarms , relative to both the study-similar and the no-load conditions .
	manualset3
163511	5	412192	7	NULL	NULL	0	NULL	no-load conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The results followed suit : The test-similar condition produced significantly elevated false alarms , relative to both the study-similar and the no-load conditions .
	manualset3
163512	1	412193	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results for mortality were based on vital statistics for the age group 40-69 years , for the periods 1966-76 and 1977-87 .
	manualset3
163513	2	412193	7	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results for mortality were based on vital statistics for the age group 40-69 years , for the periods 1966-76 and 1977-87 .
	manualset3
163514	3	412193	7	NULL	NULL	0	NULL	statistics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The results for mortality were based on vital statistics for the age group 40-69 years , for the periods 1966-76 and 1977-87 .
	manualset3
163515	4	412193	7	NULL	NULL	0	NULL	age group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results for mortality were based on vital statistics for the age group 40-69 years , for the periods 1966-76 and 1977-87 .
	manualset3
163516	5	412193	7	NULL	NULL	0	NULL	40-69 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The results for mortality were based on vital statistics for the age group 40-69 years , for the periods 1966-76 and 1977-87 .
	manualset3
163517	6	412193	7	NULL	NULL	0	NULL	periods	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The results for mortality were based on vital statistics for the age group 40-69 years , for the periods 1966-76 and 1977-87 .
	manualset3
163518	7	412193	7	NULL	NULL	0	NULL	1966-76	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The results for mortality were based on vital statistics for the age group 40-69 years , for the periods 1966-76 and 1977-87 .
	manualset3
163519	8	412193	7	NULL	NULL	0	NULL	1977-87	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The results for mortality were based on vital statistics for the age group 40-69 years , for the periods 1966-76 and 1977-87 .
	manualset3
163520	1	412194	7	NULL	NULL	NULL	NULL	 results 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results give evidence that properly folded PAF is a prerequisite for its activity .
	manualset3
163521	3	412194	7	NULL	NULL	NULL	NULL	folded PAF 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results give evidence that properly folded PAF is a prerequisite for its activity .
	manualset3
163522	2	412194	7	NULL	NULL	0	NULL	evidence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results give evidence that properly folded PAF is a prerequisite for its activity .
	manualset3
163523	4	412194	7	NULL	NULL	NULL	NULL	prerequisite	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results give evidence that properly folded PAF is a prerequisite for its activity .
	manualset3
163524	5	412194	7	NULL	NULL	NULL	NULL	activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results give evidence that properly folded PAF is a prerequisite for its activity .
	manualset3
163525	1	412195	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results give rise to the assumption that E. suis is capable of independent glucose breakdown .
	manualset3
163526	2	412195	7	NULL	NULL	NULL	NULL	assumption	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results give rise to the assumption that E. suis is capable of independent glucose breakdown .
	manualset3
163527	3	412195	7	NULL	NULL	0	NULL	E. suis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results give rise to the assumption that E. suis is capable of independent glucose breakdown .
	manualset3
163528	4	412195	7	NULL	NULL	0	NULL	 glucose breakdown 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results give rise to the assumption that E. suis is capable of independent glucose breakdown .
	manualset3
163529	1	412196	7	NULL	NULL	NULL	NULL	results 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results have been interpreted by reference to the accepted theories of steric stabilization and dispersion polymerization , and a model is proposed for the nanoparticle formation in the presence of Dextran .
	manualset3
163530	2	412196	7	NULL	NULL	0	NULL	reference	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results have been interpreted by reference to the accepted theories of steric stabilization and dispersion polymerization , and a model is proposed for the nanoparticle formation in the presence of Dextran .
	manualset3
163531	3	412196	7	NULL	NULL	NULL	NULL	steric stabilization 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results have been interpreted by reference to the accepted theories of steric stabilization and dispersion polymerization , and a model is proposed for the nanoparticle formation in the presence of Dextran .
	manualset3
163532	4	412196	7	NULL	NULL	NULL	NULL	 dispersion polymerization	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results have been interpreted by reference to the accepted theories of steric stabilization and dispersion polymerization , and a model is proposed for the nanoparticle formation in the presence of Dextran .
	manualset3
163533	5	412196	7	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The results have been interpreted by reference to the accepted theories of steric stabilization and dispersion polymerization , and a model is proposed for the nanoparticle formation in the presence of Dextran .
	manualset3
163534	6	412196	7	NULL	NULL	0	NULL	nanoparticle formation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results have been interpreted by reference to the accepted theories of steric stabilization and dispersion polymerization , and a model is proposed for the nanoparticle formation in the presence of Dextran .
	manualset3
163535	7	412196	7	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results have been interpreted by reference to the accepted theories of steric stabilization and dispersion polymerization , and a model is proposed for the nanoparticle formation in the presence of Dextran .
	manualset3
163536	8	412196	7	NULL	NULL	0	NULL	Dextran 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results have been interpreted by reference to the accepted theories of steric stabilization and dispersion polymerization , and a model is proposed for the nanoparticle formation in the presence of Dextran .
	manualset3
164583	9	412196	7	NULL	NULL	NULL	NULL	accepted theories	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results have been interpreted by reference to the accepted theories of steric stabilization and dispersion polymerization , and a model is proposed for the nanoparticle formation in the presence of Dextran .
	manualset3
163537	1	412197	7	NULL	NULL	NULL	NULL	 results 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results have demonstrated that ( 1 ) beta-amyloid peptide ( 25-35 ) , in the presence of IFN gamma or TNF alpha , induces the production of NO in the astrocyte cell line C6 , while neither cytokine was effective per se ; ( 2 ) NO generation is also synergically induced by beta-amyloid peptide ( 25-35 ) in the presence of IL-1 beta , the latter being a cytokine able to activate astrocytes per se ; ( 3 ) the effect of beta-amyloid peptide ( 25-35 ) is due to the induction of the expression of the gene of inducible NO-synthase .
	manualset3
163538	2	412197	7	NULL	NULL	0	NULL	beta-amyloid peptide ( 25-35 )	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The results have demonstrated that ( 1 ) beta-amyloid peptide ( 25-35 ) , in the presence of IFN gamma or TNF alpha , induces the production of NO in the astrocyte cell line C6 , while neither cytokine was effective per se ; ( 2 ) NO generation is also synergically induced by beta-amyloid peptide ( 25-35 ) in the presence of IL-1 beta , the latter being a cytokine able to activate astrocytes per se ; ( 3 ) the effect of beta-amyloid peptide ( 25-35 ) is due to the induction of the expression of the gene of inducible NO-synthase .
	manualset3
163539	3	412197	7	NULL	NULL	0	NULL	presence	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results have demonstrated that ( 1 ) beta-amyloid peptide ( 25-35 ) , in the presence of IFN gamma or TNF alpha , induces the production of NO in the astrocyte cell line C6 , while neither cytokine was effective per se ; ( 2 ) NO generation is also synergically induced by beta-amyloid peptide ( 25-35 ) in the presence of IL-1 beta , the latter being a cytokine able to activate astrocytes per se ; ( 3 ) the effect of beta-amyloid peptide ( 25-35 ) is due to the induction of the expression of the gene of inducible NO-synthase .
	manualset3
163540	4	412197	7	NULL	NULL	0	NULL	IFN gamma	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results have demonstrated that ( 1 ) beta-amyloid peptide ( 25-35 ) , in the presence of IFN gamma or TNF alpha , induces the production of NO in the astrocyte cell line C6 , while neither cytokine was effective per se ; ( 2 ) NO generation is also synergically induced by beta-amyloid peptide ( 25-35 ) in the presence of IL-1 beta , the latter being a cytokine able to activate astrocytes per se ; ( 3 ) the effect of beta-amyloid peptide ( 25-35 ) is due to the induction of the expression of the gene of inducible NO-synthase .
	manualset3
163541	5	412197	7	NULL	NULL	0	NULL	TNF alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results have demonstrated that ( 1 ) beta-amyloid peptide ( 25-35 ) , in the presence of IFN gamma or TNF alpha , induces the production of NO in the astrocyte cell line C6 , while neither cytokine was effective per se ; ( 2 ) NO generation is also synergically induced by beta-amyloid peptide ( 25-35 ) in the presence of IL-1 beta , the latter being a cytokine able to activate astrocytes per se ; ( 3 ) the effect of beta-amyloid peptide ( 25-35 ) is due to the induction of the expression of the gene of inducible NO-synthase .
	manualset3
163542	6	412197	7	NULL	NULL	0	NULL	production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results have demonstrated that ( 1 ) beta-amyloid peptide ( 25-35 ) , in the presence of IFN gamma or TNF alpha , induces the production of NO in the astrocyte cell line C6 , while neither cytokine was effective per se ; ( 2 ) NO generation is also synergically induced by beta-amyloid peptide ( 25-35 ) in the presence of IL-1 beta , the latter being a cytokine able to activate astrocytes per se ; ( 3 ) the effect of beta-amyloid peptide ( 25-35 ) is due to the induction of the expression of the gene of inducible NO-synthase .
	manualset3
163543	7	412197	7	NULL	NULL	0	NULL	NO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results have demonstrated that ( 1 ) beta-amyloid peptide ( 25-35 ) , in the presence of IFN gamma or TNF alpha , induces the production of NO in the astrocyte cell line C6 , while neither cytokine was effective per se ; ( 2 ) NO generation is also synergically induced by beta-amyloid peptide ( 25-35 ) in the presence of IL-1 beta , the latter being a cytokine able to activate astrocytes per se ; ( 3 ) the effect of beta-amyloid peptide ( 25-35 ) is due to the induction of the expression of the gene of inducible NO-synthase .
	manualset3
163544	8	412197	7	NULL	NULL	0	NULL	astrocyte cell line C6	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The results have demonstrated that ( 1 ) beta-amyloid peptide ( 25-35 ) , in the presence of IFN gamma or TNF alpha , induces the production of NO in the astrocyte cell line C6 , while neither cytokine was effective per se ; ( 2 ) NO generation is also synergically induced by beta-amyloid peptide ( 25-35 ) in the presence of IL-1 beta , the latter being a cytokine able to activate astrocytes per se ; ( 3 ) the effect of beta-amyloid peptide ( 25-35 ) is due to the induction of the expression of the gene of inducible NO-synthase .
	manualset3
163545	9	412197	7	NULL	NULL	0	NULL	 cytokine	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results have demonstrated that ( 1 ) beta-amyloid peptide ( 25-35 ) , in the presence of IFN gamma or TNF alpha , induces the production of NO in the astrocyte cell line C6 , while neither cytokine was effective per se ; ( 2 ) NO generation is also synergically induced by beta-amyloid peptide ( 25-35 ) in the presence of IL-1 beta , the latter being a cytokine able to activate astrocytes per se ; ( 3 ) the effect of beta-amyloid peptide ( 25-35 ) is due to the induction of the expression of the gene of inducible NO-synthase .
	manualset3
163546	10	412197	7	NULL	NULL	NULL	NULL	 NO generation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results have demonstrated that ( 1 ) beta-amyloid peptide ( 25-35 ) , in the presence of IFN gamma or TNF alpha , induces the production of NO in the astrocyte cell line C6 , while neither cytokine was effective per se ; ( 2 ) NO generation is also synergically induced by beta-amyloid peptide ( 25-35 ) in the presence of IL-1 beta , the latter being a cytokine able to activate astrocytes per se ; ( 3 ) the effect of beta-amyloid peptide ( 25-35 ) is due to the induction of the expression of the gene of inducible NO-synthase .
	manualset3
163547	11	412197	7	NULL	NULL	NULL	NULL	beta-amyloid peptide ( 25-35 )	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results have demonstrated that ( 1 ) beta-amyloid peptide ( 25-35 ) , in the presence of IFN gamma or TNF alpha , induces the production of NO in the astrocyte cell line C6 , while neither cytokine was effective per se ; ( 2 ) NO generation is also synergically induced by beta-amyloid peptide ( 25-35 ) in the presence of IL-1 beta , the latter being a cytokine able to activate astrocytes per se ; ( 3 ) the effect of beta-amyloid peptide ( 25-35 ) is due to the induction of the expression of the gene of inducible NO-synthase .
	manualset3
163548	12	412197	7	NULL	NULL	0	NULL	 presence	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results have demonstrated that ( 1 ) beta-amyloid peptide ( 25-35 ) , in the presence of IFN gamma or TNF alpha , induces the production of NO in the astrocyte cell line C6 , while neither cytokine was effective per se ; ( 2 ) NO generation is also synergically induced by beta-amyloid peptide ( 25-35 ) in the presence of IL-1 beta , the latter being a cytokine able to activate astrocytes per se ; ( 3 ) the effect of beta-amyloid peptide ( 25-35 ) is due to the induction of the expression of the gene of inducible NO-synthase .
	manualset3
163549	13	412197	7	NULL	NULL	0	NULL	IL-1 beta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results have demonstrated that ( 1 ) beta-amyloid peptide ( 25-35 ) , in the presence of IFN gamma or TNF alpha , induces the production of NO in the astrocyte cell line C6 , while neither cytokine was effective per se ; ( 2 ) NO generation is also synergically induced by beta-amyloid peptide ( 25-35 ) in the presence of IL-1 beta , the latter being a cytokine able to activate astrocytes per se ; ( 3 ) the effect of beta-amyloid peptide ( 25-35 ) is due to the induction of the expression of the gene of inducible NO-synthase .
	manualset3
163550	14	412197	7	NULL	NULL	0	NULL	cytokine	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results have demonstrated that ( 1 ) beta-amyloid peptide ( 25-35 ) , in the presence of IFN gamma or TNF alpha , induces the production of NO in the astrocyte cell line C6 , while neither cytokine was effective per se ; ( 2 ) NO generation is also synergically induced by beta-amyloid peptide ( 25-35 ) in the presence of IL-1 beta , the latter being a cytokine able to activate astrocytes per se ; ( 3 ) the effect of beta-amyloid peptide ( 25-35 ) is due to the induction of the expression of the gene of inducible NO-synthase .
	manualset3
163551	15	412197	7	NULL	NULL	NULL	NULL	 astrocytes	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results have demonstrated that ( 1 ) beta-amyloid peptide ( 25-35 ) , in the presence of IFN gamma or TNF alpha , induces the production of NO in the astrocyte cell line C6 , while neither cytokine was effective per se ; ( 2 ) NO generation is also synergically induced by beta-amyloid peptide ( 25-35 ) in the presence of IL-1 beta , the latter being a cytokine able to activate astrocytes per se ; ( 3 ) the effect of beta-amyloid peptide ( 25-35 ) is due to the induction of the expression of the gene of inducible NO-synthase .
	manualset3
163552	16	412197	7	NULL	NULL	NULL	NULL	effect 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results have demonstrated that ( 1 ) beta-amyloid peptide ( 25-35 ) , in the presence of IFN gamma or TNF alpha , induces the production of NO in the astrocyte cell line C6 , while neither cytokine was effective per se ; ( 2 ) NO generation is also synergically induced by beta-amyloid peptide ( 25-35 ) in the presence of IL-1 beta , the latter being a cytokine able to activate astrocytes per se ; ( 3 ) the effect of beta-amyloid peptide ( 25-35 ) is due to the induction of the expression of the gene of inducible NO-synthase .
	manualset3
163553	17	412197	7	NULL	NULL	0	NULL	beta-amyloid peptide ( 25-35 )	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The results have demonstrated that ( 1 ) beta-amyloid peptide ( 25-35 ) , in the presence of IFN gamma or TNF alpha , induces the production of NO in the astrocyte cell line C6 , while neither cytokine was effective per se ; ( 2 ) NO generation is also synergically induced by beta-amyloid peptide ( 25-35 ) in the presence of IL-1 beta , the latter being a cytokine able to activate astrocytes per se ; ( 3 ) the effect of beta-amyloid peptide ( 25-35 ) is due to the induction of the expression of the gene of inducible NO-synthase .
	manualset3
163554	18	412197	7	NULL	NULL	0	NULL	induction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results have demonstrated that ( 1 ) beta-amyloid peptide ( 25-35 ) , in the presence of IFN gamma or TNF alpha , induces the production of NO in the astrocyte cell line C6 , while neither cytokine was effective per se ; ( 2 ) NO generation is also synergically induced by beta-amyloid peptide ( 25-35 ) in the presence of IL-1 beta , the latter being a cytokine able to activate astrocytes per se ; ( 3 ) the effect of beta-amyloid peptide ( 25-35 ) is due to the induction of the expression of the gene of inducible NO-synthase .
	manualset3
163555	19	412197	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results have demonstrated that ( 1 ) beta-amyloid peptide ( 25-35 ) , in the presence of IFN gamma or TNF alpha , induces the production of NO in the astrocyte cell line C6 , while neither cytokine was effective per se ; ( 2 ) NO generation is also synergically induced by beta-amyloid peptide ( 25-35 ) in the presence of IL-1 beta , the latter being a cytokine able to activate astrocytes per se ; ( 3 ) the effect of beta-amyloid peptide ( 25-35 ) is due to the induction of the expression of the gene of inducible NO-synthase .
	manualset3
163556	20	412197	7	NULL	NULL	0	NULL	gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The results have demonstrated that ( 1 ) beta-amyloid peptide ( 25-35 ) , in the presence of IFN gamma or TNF alpha , induces the production of NO in the astrocyte cell line C6 , while neither cytokine was effective per se ; ( 2 ) NO generation is also synergically induced by beta-amyloid peptide ( 25-35 ) in the presence of IL-1 beta , the latter being a cytokine able to activate astrocytes per se ; ( 3 ) the effect of beta-amyloid peptide ( 25-35 ) is due to the induction of the expression of the gene of inducible NO-synthase .
	manualset3
163557	21	412197	7	NULL	NULL	0	NULL	inducible NO-synthase	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The results have demonstrated that ( 1 ) beta-amyloid peptide ( 25-35 ) , in the presence of IFN gamma or TNF alpha , induces the production of NO in the astrocyte cell line C6 , while neither cytokine was effective per se ; ( 2 ) NO generation is also synergically induced by beta-amyloid peptide ( 25-35 ) in the presence of IL-1 beta , the latter being a cytokine able to activate astrocytes per se ; ( 3 ) the effect of beta-amyloid peptide ( 25-35 ) is due to the induction of the expression of the gene of inducible NO-synthase .
	manualset3
163558	1	412198	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results highlighted an interesting correlation between therapy and degeneration into sarcoma ; more specifically , malignant transformation occurred both in patients who had not received any therapy and those who had received regular calcitonin treatment ; otherwise , no sarcoma degeneration occurred in the patients treated with bisphosphonates .
	manualset3
163559	3	412198	7	NULL	NULL	NULL	NULL	therapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results highlighted an interesting correlation between therapy and degeneration into sarcoma ; more specifically , malignant transformation occurred both in patients who had not received any therapy and those who had received regular calcitonin treatment ; otherwise , no sarcoma degeneration occurred in the patients treated with bisphosphonates .
	manualset3
163560	2	412198	7	NULL	NULL	0	NULL	 correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The results highlighted an interesting correlation between therapy and degeneration into sarcoma ; more specifically , malignant transformation occurred both in patients who had not received any therapy and those who had received regular calcitonin treatment ; otherwise , no sarcoma degeneration occurred in the patients treated with bisphosphonates .
	manualset3
163561	4	412198	7	NULL	NULL	0	NULL	degeneration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results highlighted an interesting correlation between therapy and degeneration into sarcoma ; more specifically , malignant transformation occurred both in patients who had not received any therapy and those who had received regular calcitonin treatment ; otherwise , no sarcoma degeneration occurred in the patients treated with bisphosphonates .
	manualset3
163562	5	412198	7	NULL	NULL	0	NULL	sarcoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The results highlighted an interesting correlation between therapy and degeneration into sarcoma ; more specifically , malignant transformation occurred both in patients who had not received any therapy and those who had received regular calcitonin treatment ; otherwise , no sarcoma degeneration occurred in the patients treated with bisphosphonates .
	manualset3
163563	6	412198	7	NULL	NULL	0	NULL	malignant transformation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results highlighted an interesting correlation between therapy and degeneration into sarcoma ; more specifically , malignant transformation occurred both in patients who had not received any therapy and those who had received regular calcitonin treatment ; otherwise , no sarcoma degeneration occurred in the patients treated with bisphosphonates .
	manualset3
163564	7	412198	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results highlighted an interesting correlation between therapy and degeneration into sarcoma ; more specifically , malignant transformation occurred both in patients who had not received any therapy and those who had received regular calcitonin treatment ; otherwise , no sarcoma degeneration occurred in the patients treated with bisphosphonates .
	manualset3
163565	8	412198	7	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results highlighted an interesting correlation between therapy and degeneration into sarcoma ; more specifically , malignant transformation occurred both in patients who had not received any therapy and those who had received regular calcitonin treatment ; otherwise , no sarcoma degeneration occurred in the patients treated with bisphosphonates .
	manualset3
163566	9	412198	7	NULL	NULL	NULL	NULL	calcitonin treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results highlighted an interesting correlation between therapy and degeneration into sarcoma ; more specifically , malignant transformation occurred both in patients who had not received any therapy and those who had received regular calcitonin treatment ; otherwise , no sarcoma degeneration occurred in the patients treated with bisphosphonates .
	manualset3
163567	10	412198	7	NULL	NULL	NULL	NULL	sarcoma degeneration	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results highlighted an interesting correlation between therapy and degeneration into sarcoma ; more specifically , malignant transformation occurred both in patients who had not received any therapy and those who had received regular calcitonin treatment ; otherwise , no sarcoma degeneration occurred in the patients treated with bisphosphonates .
	manualset3
163568	11	412198	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results highlighted an interesting correlation between therapy and degeneration into sarcoma ; more specifically , malignant transformation occurred both in patients who had not received any therapy and those who had received regular calcitonin treatment ; otherwise , no sarcoma degeneration occurred in the patients treated with bisphosphonates .
	manualset3
163569	12	412198	7	NULL	NULL	0	NULL	 bisphosphonates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results highlighted an interesting correlation between therapy and degeneration into sarcoma ; more specifically , malignant transformation occurred both in patients who had not received any therapy and those who had received regular calcitonin treatment ; otherwise , no sarcoma degeneration occurred in the patients treated with bisphosphonates .
	manualset3
163570	1	412199	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate good correlation between excess voltage noise , thought to reflect calcium channel activity , and insulin release evoked by changing extracellular potassium .
	manualset3
163571	2	412199	7	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate good correlation between excess voltage noise , thought to reflect calcium channel activity , and insulin release evoked by changing extracellular potassium .
	manualset3
163572	3	412199	7	NULL	NULL	0	NULL	excess voltage noise	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate good correlation between excess voltage noise , thought to reflect calcium channel activity , and insulin release evoked by changing extracellular potassium .
	manualset3
163573	4	412199	7	NULL	NULL	NULL	NULL	calcium channel activity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate good correlation between excess voltage noise , thought to reflect calcium channel activity , and insulin release evoked by changing extracellular potassium .
	manualset3
163574	5	412199	7	NULL	NULL	0	NULL	insulin release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate good correlation between excess voltage noise , thought to reflect calcium channel activity , and insulin release evoked by changing extracellular potassium .
	manualset3
163575	6	412199	7	NULL	NULL	NULL	NULL	extracellular potassium	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate good correlation between excess voltage noise , thought to reflect calcium channel activity , and insulin release evoked by changing extracellular potassium .
	manualset3
163576	1	412200	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that , although hydrogen bonding and hydrophobic interaction are both involved in the interactions between A42 and EGCG , hydrogen bonding mainly happens in A1-16 while hydrophobic interaction mainly happens in A17-42 .
	manualset3
163577	2	412200	7	NULL	NULL	0	NULL	hydrogen bonding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that , although hydrogen bonding and hydrophobic interaction are both involved in the interactions between A42 and EGCG , hydrogen bonding mainly happens in A1-16 while hydrophobic interaction mainly happens in A17-42 .
	manualset3
163578	3	412200	7	NULL	NULL	0	NULL	hydrophobic interaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that , although hydrogen bonding and hydrophobic interaction are both involved in the interactions between A42 and EGCG , hydrogen bonding mainly happens in A1-16 while hydrophobic interaction mainly happens in A17-42 .
	manualset3
163579	4	412200	7	NULL	NULL	0	NULL	 interactions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that , although hydrogen bonding and hydrophobic interaction are both involved in the interactions between A42 and EGCG , hydrogen bonding mainly happens in A1-16 while hydrophobic interaction mainly happens in A17-42 .
	manualset3
163580	5	412200	7	NULL	NULL	0	NULL	 A42	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that , although hydrogen bonding and hydrophobic interaction are both involved in the interactions between A42 and EGCG , hydrogen bonding mainly happens in A1-16 while hydrophobic interaction mainly happens in A17-42 .
	manualset3
163581	6	412200	7	NULL	NULL	0	NULL	EGCG	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that , although hydrogen bonding and hydrophobic interaction are both involved in the interactions between A42 and EGCG , hydrogen bonding mainly happens in A1-16 while hydrophobic interaction mainly happens in A17-42 .
	manualset3
163582	7	412200	7	NULL	NULL	0	NULL	hydrogen bonding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that , although hydrogen bonding and hydrophobic interaction are both involved in the interactions between A42 and EGCG , hydrogen bonding mainly happens in A1-16 while hydrophobic interaction mainly happens in A17-42 .
	manualset3
163583	8	412200	7	NULL	NULL	0	NULL	A1-16 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that , although hydrogen bonding and hydrophobic interaction are both involved in the interactions between A42 and EGCG , hydrogen bonding mainly happens in A1-16 while hydrophobic interaction mainly happens in A17-42 .
	manualset3
163584	9	412200	7	NULL	NULL	0	NULL	hydrophobic interaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that , although hydrogen bonding and hydrophobic interaction are both involved in the interactions between A42 and EGCG , hydrogen bonding mainly happens in A1-16 while hydrophobic interaction mainly happens in A17-42 .
	manualset3
163585	10	412200	7	NULL	NULL	0	NULL	A17-42	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that , although hydrogen bonding and hydrophobic interaction are both involved in the interactions between A42 and EGCG , hydrogen bonding mainly happens in A1-16 while hydrophobic interaction mainly happens in A17-42 .
	manualset3
163586	1	412201	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that CHP-induced hypothermia is mediated by cholinergic stimulation of heat loss pathways in CNS thermoregulatory centers .
	manualset3
163587	2	412201	7	NULL	NULL	0	NULL	CHP-induced hypothermia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that CHP-induced hypothermia is mediated by cholinergic stimulation of heat loss pathways in CNS thermoregulatory centers .
	manualset3
163588	3	412201	7	NULL	NULL	NULL	NULL	cholinergic stimulation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that CHP-induced hypothermia is mediated by cholinergic stimulation of heat loss pathways in CNS thermoregulatory centers .
	manualset3
163589	4	412201	7	NULL	NULL	NULL	NULL	 heat loss pathways	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that CHP-induced hypothermia is mediated by cholinergic stimulation of heat loss pathways in CNS thermoregulatory centers .
	manualset3
163590	5	412201	7	NULL	NULL	0	NULL	CNS thermoregulatory centers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that CHP-induced hypothermia is mediated by cholinergic stimulation of heat loss pathways in CNS thermoregulatory centers .
	manualset3
163591	1	412202	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that HBeAg is found constantly in the early phase of acute hepatitis B. The presence of HBeAg for more than 10 weeks after the onset of symptoms seems to be of prognostic value and signifies the development of a chronic HBsAg carrier state .
	manualset3
163592	2	412202	7	NULL	NULL	0	NULL	HBeAg	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that HBeAg is found constantly in the early phase of acute hepatitis B. The presence of HBeAg for more than 10 weeks after the onset of symptoms seems to be of prognostic value and signifies the development of a chronic HBsAg carrier state .
	manualset3
163593	3	412202	7	NULL	NULL	0	NULL	early phase	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that HBeAg is found constantly in the early phase of acute hepatitis B. The presence of HBeAg for more than 10 weeks after the onset of symptoms seems to be of prognostic value and signifies the development of a chronic HBsAg carrier state .
	manualset3
163594	4	412202	7	NULL	NULL	0	NULL	acute hepatitis B	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that HBeAg is found constantly in the early phase of acute hepatitis B. The presence of HBeAg for more than 10 weeks after the onset of symptoms seems to be of prognostic value and signifies the development of a chronic HBsAg carrier state .
	manualset3
163595	5	412202	7	NULL	NULL	0	NULL	presence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that HBeAg is found constantly in the early phase of acute hepatitis B. The presence of HBeAg for more than 10 weeks after the onset of symptoms seems to be of prognostic value and signifies the development of a chronic HBsAg carrier state .
	manualset3
163596	6	412202	7	NULL	NULL	0	NULL	HBeAg	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that HBeAg is found constantly in the early phase of acute hepatitis B. The presence of HBeAg for more than 10 weeks after the onset of symptoms seems to be of prognostic value and signifies the development of a chronic HBsAg carrier state .
	manualset3
163597	7	412202	7	NULL	NULL	0	NULL	10 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that HBeAg is found constantly in the early phase of acute hepatitis B. The presence of HBeAg for more than 10 weeks after the onset of symptoms seems to be of prognostic value and signifies the development of a chronic HBsAg carrier state .
	manualset3
163598	8	412202	7	NULL	NULL	0	NULL	onset	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that HBeAg is found constantly in the early phase of acute hepatitis B. The presence of HBeAg for more than 10 weeks after the onset of symptoms seems to be of prognostic value and signifies the development of a chronic HBsAg carrier state .
	manualset3
163599	9	412202	7	NULL	NULL	0	NULL	symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that HBeAg is found constantly in the early phase of acute hepatitis B. The presence of HBeAg for more than 10 weeks after the onset of symptoms seems to be of prognostic value and signifies the development of a chronic HBsAg carrier state .
	manualset3
163600	10	412202	7	NULL	NULL	0	NULL	prognostic value	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that HBeAg is found constantly in the early phase of acute hepatitis B. The presence of HBeAg for more than 10 weeks after the onset of symptoms seems to be of prognostic value and signifies the development of a chronic HBsAg carrier state .
	manualset3
163601	11	412202	7	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that HBeAg is found constantly in the early phase of acute hepatitis B. The presence of HBeAg for more than 10 weeks after the onset of symptoms seems to be of prognostic value and signifies the development of a chronic HBsAg carrier state .
	manualset3
163602	12	412202	7	NULL	NULL	NULL	NULL	chronic HBsAg carrier state	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that HBeAg is found constantly in the early phase of acute hepatitis B. The presence of HBeAg for more than 10 weeks after the onset of symptoms seems to be of prognostic value and signifies the development of a chronic HBsAg carrier state .
	manualset3
163603	1	412203	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that antibiotic-induced hypoprothrombinemia in vivo is not caused by inhibition of enzymes of the gamma-carboxylation system , such as vitamin K reductase and gamma-glutamylcarboxylase , but is related to the endogenous vitamin K level .
	manualset3
163604	2	412203	7	NULL	NULL	0	NULL	antibiotic-induced hypoprothrombinemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that antibiotic-induced hypoprothrombinemia in vivo is not caused by inhibition of enzymes of the gamma-carboxylation system , such as vitamin K reductase and gamma-glutamylcarboxylase , but is related to the endogenous vitamin K level .
	manualset3
163605	3	412203	7	NULL	NULL	0	NULL	inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that antibiotic-induced hypoprothrombinemia in vivo is not caused by inhibition of enzymes of the gamma-carboxylation system , such as vitamin K reductase and gamma-glutamylcarboxylase , but is related to the endogenous vitamin K level .
	manualset3
163606	4	412203	7	NULL	NULL	0	NULL	enzymes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that antibiotic-induced hypoprothrombinemia in vivo is not caused by inhibition of enzymes of the gamma-carboxylation system , such as vitamin K reductase and gamma-glutamylcarboxylase , but is related to the endogenous vitamin K level .
	manualset3
163607	5	412203	7	NULL	NULL	0	NULL	gamma-carboxylation system	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that antibiotic-induced hypoprothrombinemia in vivo is not caused by inhibition of enzymes of the gamma-carboxylation system , such as vitamin K reductase and gamma-glutamylcarboxylase , but is related to the endogenous vitamin K level .
	manualset3
163608	6	412203	7	NULL	NULL	0	NULL	vitamin K reductase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that antibiotic-induced hypoprothrombinemia in vivo is not caused by inhibition of enzymes of the gamma-carboxylation system , such as vitamin K reductase and gamma-glutamylcarboxylase , but is related to the endogenous vitamin K level .
	manualset3
163609	7	412203	7	NULL	NULL	0	NULL	gamma-glutamylcarboxylase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that antibiotic-induced hypoprothrombinemia in vivo is not caused by inhibition of enzymes of the gamma-carboxylation system , such as vitamin K reductase and gamma-glutamylcarboxylase , but is related to the endogenous vitamin K level .
	manualset3
163610	8	412203	7	NULL	NULL	0	NULL	endogenous vitamin K level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that antibiotic-induced hypoprothrombinemia in vivo is not caused by inhibition of enzymes of the gamma-carboxylation system , such as vitamin K reductase and gamma-glutamylcarboxylase , but is related to the endogenous vitamin K level .
	manualset3
163611	1	412204	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that in Down 's fibroblasts the mechanisms controlling APP release are at least quantitatively altered .
	manualset3
163612	2	412204	7	NULL	NULL	0	NULL	Down 's fibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that in Down 's fibroblasts the mechanisms controlling APP release are at least quantitatively altered .
	manualset3
163613	3	412204	7	NULL	NULL	NULL	NULL	mechanisms	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that in Down 's fibroblasts the mechanisms controlling APP release are at least quantitatively altered .
	manualset3
163614	4	412204	7	NULL	NULL	NULL	NULL	APP release	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that in Down 's fibroblasts the mechanisms controlling APP release are at least quantitatively altered .
	manualset3
163615	1	412205	7	NULL	NULL	NULL	NULL	results 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that opportunities exist to simplify antihypertensive therapy by using current ambulatory PRA levels to guide drug selections and subtractions .
	manualset3
163616	2	412205	7	NULL	NULL	0	NULL	opportunities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that opportunities exist to simplify antihypertensive therapy by using current ambulatory PRA levels to guide drug selections and subtractions .
	manualset3
163617	3	412205	7	NULL	NULL	0	NULL	antihypertensive therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that opportunities exist to simplify antihypertensive therapy by using current ambulatory PRA levels to guide drug selections and subtractions .
	manualset3
163618	4	412205	7	NULL	NULL	NULL	NULL	current ambulatory PRA levels 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that opportunities exist to simplify antihypertensive therapy by using current ambulatory PRA levels to guide drug selections and subtractions .
	manualset3
163619	5	412205	7	NULL	NULL	0	NULL	drug selections	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that opportunities exist to simplify antihypertensive therapy by using current ambulatory PRA levels to guide drug selections and subtractions .
	manualset3
163620	6	412205	7	NULL	NULL	0	NULL	 subtractions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that opportunities exist to simplify antihypertensive therapy by using current ambulatory PRA levels to guide drug selections and subtractions .
	manualset3
163621	1	412206	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that pulmonary instillation of small volumes of iodinated nanoparticles could be successfully used to aid staging of lung cancer by CT imaging .
	manualset3
163622	2	412206	7	NULL	NULL	0	NULL	pulmonary instillation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that pulmonary instillation of small volumes of iodinated nanoparticles could be successfully used to aid staging of lung cancer by CT imaging .
	manualset3
163623	3	412206	7	NULL	NULL	0	NULL	small volumes 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that pulmonary instillation of small volumes of iodinated nanoparticles could be successfully used to aid staging of lung cancer by CT imaging .
	manualset3
163624	4	412206	7	NULL	NULL	NULL	NULL	iodinated nanoparticles	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that pulmonary instillation of small volumes of iodinated nanoparticles could be successfully used to aid staging of lung cancer by CT imaging .
	manualset3
163625	5	412206	7	NULL	NULL	NULL	NULL	lung cancer	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that pulmonary instillation of small volumes of iodinated nanoparticles could be successfully used to aid staging of lung cancer by CT imaging .
	manualset3
163626	6	412206	7	NULL	NULL	NULL	NULL	CT imaging	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that pulmonary instillation of small volumes of iodinated nanoparticles could be successfully used to aid staging of lung cancer by CT imaging .
	manualset3
163628	1	412207	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that short-term treatment with 1 , 000 micrograms.day-1 BDP reduces bronchial hyperreactivity ( BHR ) in asthmatic patients , whilst having subtle effects on HPA axis .
	manualset3
163629	2	412207	7	NULL	NULL	0	NULL	short-term treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that short-term treatment with 1 , 000 micrograms.day-1 BDP reduces bronchial hyperreactivity ( BHR ) in asthmatic patients , whilst having subtle effects on HPA axis .
	manualset3
163630	3	412207	7	NULL	NULL	NULL	NULL	1 , 000 micrograms.day-1	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that short-term treatment with 1 , 000 micrograms.day-1 BDP reduces bronchial hyperreactivity ( BHR ) in asthmatic patients , whilst having subtle effects on HPA axis .
	manualset3
163631	4	412207	7	NULL	NULL	0	NULL	BDP	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that short-term treatment with 1 , 000 micrograms.day-1 BDP reduces bronchial hyperreactivity ( BHR ) in asthmatic patients , whilst having subtle effects on HPA axis .
	manualset3
163632	5	412207	7	NULL	NULL	0	NULL	 bronchial hyperreactivity ( BHR )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that short-term treatment with 1 , 000 micrograms.day-1 BDP reduces bronchial hyperreactivity ( BHR ) in asthmatic patients , whilst having subtle effects on HPA axis .
	manualset3
163633	6	412207	7	NULL	NULL	0	NULL	asthmatic patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that short-term treatment with 1 , 000 micrograms.day-1 BDP reduces bronchial hyperreactivity ( BHR ) in asthmatic patients , whilst having subtle effects on HPA axis .
	manualset3
163635	7	412207	7	NULL	NULL	NULL	NULL	HPA axis	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that short-term treatment with 1 , 000 micrograms.day-1 BDP reduces bronchial hyperreactivity ( BHR ) in asthmatic patients , whilst having subtle effects on HPA axis .
	manualset3
163636	1	412208	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that the SPF value was related to both a photo-reaction and a biological reaction .
	manualset3
163637	2	412208	7	NULL	NULL	0	NULL	SPF value 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that the SPF value was related to both a photo-reaction and a biological reaction .
	manualset3
163638	3	412208	7	NULL	NULL	0	NULL	photo-reaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that the SPF value was related to both a photo-reaction and a biological reaction .
	manualset3
163639	4	412208	7	NULL	NULL	0	NULL	biological reaction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that the SPF value was related to both a photo-reaction and a biological reaction .
	manualset3
163640	1	412209	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that the cell group is distinguished by massive projections to parasympathetic preganglionic neurons in the brainstem ( especially in the salivatory nuclei and dorsal motor nucleus of the vagus nerve ) and to parts of the parabrachial nucleus and nucleus of the solitary tract that relay viscerosensory and gustatory information .
	manualset3
163641	2	412209	7	NULL	NULL	0	NULL	cell group	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that the cell group is distinguished by massive projections to parasympathetic preganglionic neurons in the brainstem ( especially in the salivatory nuclei and dorsal motor nucleus of the vagus nerve ) and to parts of the parabrachial nucleus and nucleus of the solitary tract that relay viscerosensory and gustatory information .
	manualset3
163642	3	412209	7	NULL	NULL	NULL	NULL	massive projections 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that the cell group is distinguished by massive projections to parasympathetic preganglionic neurons in the brainstem ( especially in the salivatory nuclei and dorsal motor nucleus of the vagus nerve ) and to parts of the parabrachial nucleus and nucleus of the solitary tract that relay viscerosensory and gustatory information .
	manualset3
163643	4	412209	7	NULL	NULL	0	NULL	parasympathetic preganglionic neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that the cell group is distinguished by massive projections to parasympathetic preganglionic neurons in the brainstem ( especially in the salivatory nuclei and dorsal motor nucleus of the vagus nerve ) and to parts of the parabrachial nucleus and nucleus of the solitary tract that relay viscerosensory and gustatory information .
	manualset3
163644	5	412209	7	NULL	NULL	0	NULL	brainstem 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that the cell group is distinguished by massive projections to parasympathetic preganglionic neurons in the brainstem ( especially in the salivatory nuclei and dorsal motor nucleus of the vagus nerve ) and to parts of the parabrachial nucleus and nucleus of the solitary tract that relay viscerosensory and gustatory information .
	manualset3
163645	6	412209	7	NULL	NULL	NULL	NULL	salivatory nuclei 	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that the cell group is distinguished by massive projections to parasympathetic preganglionic neurons in the brainstem ( especially in the salivatory nuclei and dorsal motor nucleus of the vagus nerve ) and to parts of the parabrachial nucleus and nucleus of the solitary tract that relay viscerosensory and gustatory information .
	manualset3
163646	7	412209	7	NULL	NULL	NULL	NULL	dorsal motor nucleus 	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that the cell group is distinguished by massive projections to parasympathetic preganglionic neurons in the brainstem ( especially in the salivatory nuclei and dorsal motor nucleus of the vagus nerve ) and to parts of the parabrachial nucleus and nucleus of the solitary tract that relay viscerosensory and gustatory information .
	manualset3
163647	8	412209	7	NULL	NULL	0	NULL	 vagus nerve	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that the cell group is distinguished by massive projections to parasympathetic preganglionic neurons in the brainstem ( especially in the salivatory nuclei and dorsal motor nucleus of the vagus nerve ) and to parts of the parabrachial nucleus and nucleus of the solitary tract that relay viscerosensory and gustatory information .
	manualset3
163648	9	412209	7	NULL	NULL	NULL	NULL	parabrachial nucleus 	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that the cell group is distinguished by massive projections to parasympathetic preganglionic neurons in the brainstem ( especially in the salivatory nuclei and dorsal motor nucleus of the vagus nerve ) and to parts of the parabrachial nucleus and nucleus of the solitary tract that relay viscerosensory and gustatory information .
	manualset3
163649	10	412209	7	NULL	NULL	0	NULL	nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that the cell group is distinguished by massive projections to parasympathetic preganglionic neurons in the brainstem ( especially in the salivatory nuclei and dorsal motor nucleus of the vagus nerve ) and to parts of the parabrachial nucleus and nucleus of the solitary tract that relay viscerosensory and gustatory information .
	manualset3
163650	11	412209	7	NULL	NULL	0	NULL	solitary tract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that the cell group is distinguished by massive projections to parasympathetic preganglionic neurons in the brainstem ( especially in the salivatory nuclei and dorsal motor nucleus of the vagus nerve ) and to parts of the parabrachial nucleus and nucleus of the solitary tract that relay viscerosensory and gustatory information .
	manualset3
163651	12	412209	7	NULL	NULL	0	NULL	viscerosensory information	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that the cell group is distinguished by massive projections to parasympathetic preganglionic neurons in the brainstem ( especially in the salivatory nuclei and dorsal motor nucleus of the vagus nerve ) and to parts of the parabrachial nucleus and nucleus of the solitary tract that relay viscerosensory and gustatory information .
	manualset3
163652	13	412209	7	NULL	NULL	0	NULL	gustatory information	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that the cell group is distinguished by massive projections to parasympathetic preganglionic neurons in the brainstem ( especially in the salivatory nuclei and dorsal motor nucleus of the vagus nerve ) and to parts of the parabrachial nucleus and nucleus of the solitary tract that relay viscerosensory and gustatory information .
	manualset3
163653	1	412210	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that the in vitro system developed on endometrial capillaries derived from human decidua provides a stable low background of DNA synthesis against which small amounts of possible mediators of endothelial mitoses , e.g. estradiol , progesterone and various synthetic progestogens , can be tested .
	manualset3
163654	2	412210	7	NULL	NULL	0	NULL	in vitro system	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that the in vitro system developed on endometrial capillaries derived from human decidua provides a stable low background of DNA synthesis against which small amounts of possible mediators of endothelial mitoses , e.g. estradiol , progesterone and various synthetic progestogens , can be tested .
	manualset3
163655	3	412210	7	NULL	NULL	0	NULL	endometrial capillaries	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that the in vitro system developed on endometrial capillaries derived from human decidua provides a stable low background of DNA synthesis against which small amounts of possible mediators of endothelial mitoses , e.g. estradiol , progesterone and various synthetic progestogens , can be tested .
	manualset3
163656	4	412210	7	NULL	NULL	0	NULL	human decidua	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that the in vitro system developed on endometrial capillaries derived from human decidua provides a stable low background of DNA synthesis against which small amounts of possible mediators of endothelial mitoses , e.g. estradiol , progesterone and various synthetic progestogens , can be tested .
	manualset3
163657	5	412210	7	NULL	NULL	0	NULL	DNA synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that the in vitro system developed on endometrial capillaries derived from human decidua provides a stable low background of DNA synthesis against which small amounts of possible mediators of endothelial mitoses , e.g. estradiol , progesterone and various synthetic progestogens , can be tested .
	manualset3
163658	6	412210	7	NULL	NULL	0	NULL	small amounts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that the in vitro system developed on endometrial capillaries derived from human decidua provides a stable low background of DNA synthesis against which small amounts of possible mediators of endothelial mitoses , e.g. estradiol , progesterone and various synthetic progestogens , can be tested .
	manualset3
163659	7	412210	7	NULL	NULL	0	NULL	mediators	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that the in vitro system developed on endometrial capillaries derived from human decidua provides a stable low background of DNA synthesis against which small amounts of possible mediators of endothelial mitoses , e.g. estradiol , progesterone and various synthetic progestogens , can be tested .
	manualset3
163660	8	412210	7	NULL	NULL	0	NULL	 endothelial mitoses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that the in vitro system developed on endometrial capillaries derived from human decidua provides a stable low background of DNA synthesis against which small amounts of possible mediators of endothelial mitoses , e.g. estradiol , progesterone and various synthetic progestogens , can be tested .
	manualset3
163661	9	412210	7	NULL	NULL	0	NULL	estradiol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that the in vitro system developed on endometrial capillaries derived from human decidua provides a stable low background of DNA synthesis against which small amounts of possible mediators of endothelial mitoses , e.g. estradiol , progesterone and various synthetic progestogens , can be tested .
	manualset3
163662	10	412210	7	NULL	NULL	0	NULL	progesterone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that the in vitro system developed on endometrial capillaries derived from human decidua provides a stable low background of DNA synthesis against which small amounts of possible mediators of endothelial mitoses , e.g. estradiol , progesterone and various synthetic progestogens , can be tested .
	manualset3
163663	11	412210	7	NULL	NULL	0	NULL	synthetic progestogens	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that the in vitro system developed on endometrial capillaries derived from human decidua provides a stable low background of DNA synthesis against which small amounts of possible mediators of endothelial mitoses , e.g. estradiol , progesterone and various synthetic progestogens , can be tested .
	manualset3
169730	12	412210	7	NULL	NULL	0	NULL	stable low background	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that the in vitro system developed on endometrial capillaries derived from human decidua provides a stable low background of DNA synthesis against which small amounts of possible mediators of endothelial mitoses , e.g. estradiol , progesterone and various synthetic progestogens , can be tested .
	manualset3
163664	1	412211	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that the oxygen uptake in the chronic ischaemic kidney is more decreased than its blood flow .
	manualset3
163665	2	412211	7	NULL	NULL	0	NULL	oxygen uptake 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that the oxygen uptake in the chronic ischaemic kidney is more decreased than its blood flow .
	manualset3
163666	3	412211	7	NULL	NULL	0	NULL	chronic ischaemic kidney	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that the oxygen uptake in the chronic ischaemic kidney is more decreased than its blood flow .
	manualset3
163667	4	412211	7	NULL	NULL	0	NULL	blood flow	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that the oxygen uptake in the chronic ischaemic kidney is more decreased than its blood flow .
	manualset3
163668	1	412212	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that the reminiscence bump can also be identified outside the autobiographical memory domain .
	manualset3
163669	2	412212	7	NULL	NULL	0	NULL	reminiscence bump	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that the reminiscence bump can also be identified outside the autobiographical memory domain .
	manualset3
163670	3	412212	7	NULL	NULL	0	NULL	autobiographical memory domain	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that the reminiscence bump can also be identified outside the autobiographical memory domain .
	manualset3
163671	1	412213	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that this selective extraction technology was effective for the extraction and separation of Fe , Mn oxides and OMs in the SSs , and important for further mechanism study of trace metal adsorption onto SSs .
	manualset3
163672	2	412213	7	NULL	NULL	0	NULL	selective extraction technology	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that this selective extraction technology was effective for the extraction and separation of Fe , Mn oxides and OMs in the SSs , and important for further mechanism study of trace metal adsorption onto SSs .
	manualset3
163673	3	412213	7	NULL	NULL	0	NULL	 extraction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that this selective extraction technology was effective for the extraction and separation of Fe , Mn oxides and OMs in the SSs , and important for further mechanism study of trace metal adsorption onto SSs .
	manualset3
163674	4	412213	7	NULL	NULL	0	NULL	separation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that this selective extraction technology was effective for the extraction and separation of Fe , Mn oxides and OMs in the SSs , and important for further mechanism study of trace metal adsorption onto SSs .
	manualset3
163675	5	412213	7	NULL	NULL	0	NULL	Fe 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that this selective extraction technology was effective for the extraction and separation of Fe , Mn oxides and OMs in the SSs , and important for further mechanism study of trace metal adsorption onto SSs .
	manualset3
163676	6	412213	7	NULL	NULL	0	NULL	Mn oxides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that this selective extraction technology was effective for the extraction and separation of Fe , Mn oxides and OMs in the SSs , and important for further mechanism study of trace metal adsorption onto SSs .
	manualset3
163677	7	412213	7	NULL	NULL	0	NULL	OMs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that this selective extraction technology was effective for the extraction and separation of Fe , Mn oxides and OMs in the SSs , and important for further mechanism study of trace metal adsorption onto SSs .
	manualset3
163678	8	412213	7	NULL	NULL	0	NULL	SSs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that this selective extraction technology was effective for the extraction and separation of Fe , Mn oxides and OMs in the SSs , and important for further mechanism study of trace metal adsorption onto SSs .
	manualset3
163679	9	412213	7	NULL	NULL	NULL	NULL	mechanism study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that this selective extraction technology was effective for the extraction and separation of Fe , Mn oxides and OMs in the SSs , and important for further mechanism study of trace metal adsorption onto SSs .
	manualset3
163681	11	412213	7	NULL	NULL	0	NULL	trace metal	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that this selective extraction technology was effective for the extraction and separation of Fe , Mn oxides and OMs in the SSs , and important for further mechanism study of trace metal adsorption onto SSs .
	manualset3
163682	12	412213	7	NULL	NULL	0	NULL	adsorption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that this selective extraction technology was effective for the extraction and separation of Fe , Mn oxides and OMs in the SSs , and important for further mechanism study of trace metal adsorption onto SSs .
	manualset3
163683	13	412213	7	NULL	NULL	0	NULL	SSs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that this selective extraction technology was effective for the extraction and separation of Fe , Mn oxides and OMs in the SSs , and important for further mechanism study of trace metal adsorption onto SSs .
	manualset3
163684	1	412214	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that virus-specific , cloned CTL that stably express cytolytic activity are representative of the heterogeneous populations from which they are derived and further suggest a qualitative difference in the regulation and expression of cytolytic machinery between heterogeneous populations of influenza-specific CTL and alloreactive CTL .
	manualset3
163685	2	412214	7	NULL	NULL	NULL	NULL	virus-specific,cloned CTL	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate that virus-specific , cloned CTL that stably express cytolytic activity are representative of the heterogeneous populations from which they are derived and further suggest a qualitative difference in the regulation and expression of cytolytic machinery between heterogeneous populations of influenza-specific CTL and alloreactive CTL .
	manualset3
163686	3	412214	7	NULL	NULL	0	NULL	cytolytic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that virus-specific , cloned CTL that stably express cytolytic activity are representative of the heterogeneous populations from which they are derived and further suggest a qualitative difference in the regulation and expression of cytolytic machinery between heterogeneous populations of influenza-specific CTL and alloreactive CTL .
	manualset3
163687	4	412214	7	NULL	NULL	0	NULL	heterogeneous populations	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that virus-specific , cloned CTL that stably express cytolytic activity are representative of the heterogeneous populations from which they are derived and further suggest a qualitative difference in the regulation and expression of cytolytic machinery between heterogeneous populations of influenza-specific CTL and alloreactive CTL .
	manualset3
163688	5	412214	7	NULL	NULL	0	NULL	 regulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that virus-specific , cloned CTL that stably express cytolytic activity are representative of the heterogeneous populations from which they are derived and further suggest a qualitative difference in the regulation and expression of cytolytic machinery between heterogeneous populations of influenza-specific CTL and alloreactive CTL .
	manualset3
163689	6	412214	7	NULL	NULL	0	NULL	expression 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that virus-specific , cloned CTL that stably express cytolytic activity are representative of the heterogeneous populations from which they are derived and further suggest a qualitative difference in the regulation and expression of cytolytic machinery between heterogeneous populations of influenza-specific CTL and alloreactive CTL .
	manualset3
163690	7	412214	7	NULL	NULL	0	NULL	cytolytic machinery	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that virus-specific , cloned CTL that stably express cytolytic activity are representative of the heterogeneous populations from which they are derived and further suggest a qualitative difference in the regulation and expression of cytolytic machinery between heterogeneous populations of influenza-specific CTL and alloreactive CTL .
	manualset3
163691	8	412214	7	NULL	NULL	0	NULL	heterogeneous populations	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that virus-specific , cloned CTL that stably express cytolytic activity are representative of the heterogeneous populations from which they are derived and further suggest a qualitative difference in the regulation and expression of cytolytic machinery between heterogeneous populations of influenza-specific CTL and alloreactive CTL .
	manualset3
163692	9	412214	7	NULL	NULL	0	NULL	influenza-specific CTL	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that virus-specific , cloned CTL that stably express cytolytic activity are representative of the heterogeneous populations from which they are derived and further suggest a qualitative difference in the regulation and expression of cytolytic machinery between heterogeneous populations of influenza-specific CTL and alloreactive CTL .
	manualset3
163693	10	412214	7	NULL	NULL	0	NULL	alloreactive CTL	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that virus-specific , cloned CTL that stably express cytolytic activity are representative of the heterogeneous populations from which they are derived and further suggest a qualitative difference in the regulation and expression of cytolytic machinery between heterogeneous populations of influenza-specific CTL and alloreactive CTL .
	manualset3
169731	11	412214	7	NULL	NULL	0	NULL	qualitative difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate that virus-specific , cloned CTL that stably express cytolytic activity are representative of the heterogeneous populations from which they are derived and further suggest a qualitative difference in the regulation and expression of cytolytic machinery between heterogeneous populations of influenza-specific CTL and alloreactive CTL .
	manualset3
163694	1	412215	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate the MTX is cleared from the plasma at a rate of 84.6 mL/min/m2 .
	manualset3
163695	2	412215	7	NULL	NULL	0	NULL	MTX	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate the MTX is cleared from the plasma at a rate of 84.6 mL/min/m2 .
	manualset3
163696	3	412215	7	NULL	NULL	0	NULL	plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate the MTX is cleared from the plasma at a rate of 84.6 mL/min/m2 .
	manualset3
163697	4	412215	7	NULL	NULL	0	NULL	 rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate the MTX is cleared from the plasma at a rate of 84.6 mL/min/m2 .
	manualset3
163698	5	412215	7	NULL	NULL	0	NULL	84.6 mL/min/m2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate the MTX is cleared from the plasma at a rate of 84.6 mL/min/m2 .
	manualset3
163699	1	412216	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate the potential of ticks in modulating the cytokine network of their vertebrate hosts , possibly to facilitate blood feeding .
	manualset3
163700	2	412216	7	NULL	NULL	0	NULL	potential	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate the potential of ticks in modulating the cytokine network of their vertebrate hosts , possibly to facilitate blood feeding .
	manualset3
163701	3	412216	7	NULL	NULL	0	NULL	ticks	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate the potential of ticks in modulating the cytokine network of their vertebrate hosts , possibly to facilitate blood feeding .
	manualset3
163702	4	412216	7	NULL	NULL	0	NULL	cytokine network	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate the potential of ticks in modulating the cytokine network of their vertebrate hosts , possibly to facilitate blood feeding .
	manualset3
163703	5	412216	7	NULL	NULL	0	NULL	vertebrate hosts	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate the potential of ticks in modulating the cytokine network of their vertebrate hosts , possibly to facilitate blood feeding .
	manualset3
163704	6	412216	7	NULL	NULL	0	NULL	blood feeding	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate the potential of ticks in modulating the cytokine network of their vertebrate hosts , possibly to facilitate blood feeding .
	manualset3
163705	1	412217	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate the presence of multiple anthelmintic resistance in this strain of H. contortus on this farm .
	manualset3
163706	2	412217	7	NULL	NULL	NULL	NULL	 presence	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicate the presence of multiple anthelmintic resistance in this strain of H. contortus on this farm .
	manualset3
163707	3	412217	7	NULL	NULL	0	NULL	multiple anthelmintic resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate the presence of multiple anthelmintic resistance in this strain of H. contortus on this farm .
	manualset3
163708	4	412217	7	NULL	NULL	0	NULL	strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate the presence of multiple anthelmintic resistance in this strain of H. contortus on this farm .
	manualset3
163709	5	412217	7	NULL	NULL	0	NULL	H. contortus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate the presence of multiple anthelmintic resistance in this strain of H. contortus on this farm .
	manualset3
164584	6	412217	7	NULL	NULL	0	NULL	farm	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicate the presence of multiple anthelmintic resistance in this strain of H. contortus on this farm .
	manualset3
163710	1	412218	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicated that VO ( 2 ) peak was significantly lower in obese boys compared with normal weight counterparts when the data were expressed either in conventional ratio unit ( ml ( -1 ) .
	manualset3
163711	2	412218	7	NULL	NULL	0	NULL	 VO ( 2 ) peak	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that VO ( 2 ) peak was significantly lower in obese boys compared with normal weight counterparts when the data were expressed either in conventional ratio unit ( ml ( -1 ) .
	manualset3
163712	3	412218	7	NULL	NULL	0	NULL	obese boys	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that VO ( 2 ) peak was significantly lower in obese boys compared with normal weight counterparts when the data were expressed either in conventional ratio unit ( ml ( -1 ) .
	manualset3
163713	4	412218	7	NULL	NULL	0	NULL	normal weight counterparts	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that VO ( 2 ) peak was significantly lower in obese boys compared with normal weight counterparts when the data were expressed either in conventional ratio unit ( ml ( -1 ) .
	manualset3
163714	5	412218	7	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that VO ( 2 ) peak was significantly lower in obese boys compared with normal weight counterparts when the data were expressed either in conventional ratio unit ( ml ( -1 ) .
	manualset3
163715	6	412218	7	NULL	NULL	0	NULL	conventional ratio unit 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that VO ( 2 ) peak was significantly lower in obese boys compared with normal weight counterparts when the data were expressed either in conventional ratio unit ( ml ( -1 ) .
	manualset3
163716	7	412218	7	NULL	NULL	0	NULL	( ml ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that VO ( 2 ) peak was significantly lower in obese boys compared with normal weight counterparts when the data were expressed either in conventional ratio unit ( ml ( -1 ) .
	manualset3
163717	1	412219	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicated that catalpol prevented the MPP ( + ) - induced inhibition of complex I activity and the loss of mitochondrial membrane potential .
	manualset3
163718	2	412219	7	NULL	NULL	0	NULL	catalpol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that catalpol prevented the MPP ( + ) - induced inhibition of complex I activity and the loss of mitochondrial membrane potential .
	manualset3
163719	3	412219	7	NULL	NULL	NULL	NULL	MPP ( + ) - induced inhibition	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicated that catalpol prevented the MPP ( + ) - induced inhibition of complex I activity and the loss of mitochondrial membrane potential .
	manualset3
163720	4	412219	7	NULL	NULL	NULL	NULL	complex I activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicated that catalpol prevented the MPP ( + ) - induced inhibition of complex I activity and the loss of mitochondrial membrane potential .
	manualset3
163721	5	412219	7	NULL	NULL	NULL	NULL	loss	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicated that catalpol prevented the MPP ( + ) - induced inhibition of complex I activity and the loss of mitochondrial membrane potential .
	manualset3
163722	6	412219	7	NULL	NULL	0	NULL	mitochondrial membrane potential	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that catalpol prevented the MPP ( + ) - induced inhibition of complex I activity and the loss of mitochondrial membrane potential .
	manualset3
163723	1	412220	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicated that the BsmI polymorphism is associated with increased risk of T1DM ( BB+B b vs. bb : OR = 1.30 , 95 % CI = 1.03-1 .63 ) , while the FokI , ApaI and TaqI polymorphisms were not .
	manualset3
163724	2	412220	7	NULL	NULL	0	NULL	BsmI polymorphism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the BsmI polymorphism is associated with increased risk of T1DM ( BB+B b vs. bb : OR = 1.30 , 95 % CI = 1.03-1 .63 ) , while the FokI , ApaI and TaqI polymorphisms were not .
	manualset3
163725	3	412220	7	NULL	NULL	0	NULL	increased risk	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the BsmI polymorphism is associated with increased risk of T1DM ( BB+B b vs. bb : OR = 1.30 , 95 % CI = 1.03-1 .63 ) , while the FokI , ApaI and TaqI polymorphisms were not .
	manualset3
163726	4	412220	7	NULL	NULL	0	NULL	T1DM	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the BsmI polymorphism is associated with increased risk of T1DM ( BB+B b vs. bb : OR = 1.30 , 95 % CI = 1.03-1 .63 ) , while the FokI , ApaI and TaqI polymorphisms were not .
	manualset3
163727	5	412220	7	NULL	NULL	0	NULL	BB+B b vs. bb	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the BsmI polymorphism is associated with increased risk of T1DM ( BB+B b vs. bb : OR = 1.30 , 95 % CI = 1.03-1 .63 ) , while the FokI , ApaI and TaqI polymorphisms were not .
	manualset3
163728	6	412220	7	NULL	NULL	0	NULL	OR = 1.30 , 95 % CI = 1.03-1 .63 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the BsmI polymorphism is associated with increased risk of T1DM ( BB+B b vs. bb : OR = 1.30 , 95 % CI = 1.03-1 .63 ) , while the FokI , ApaI and TaqI polymorphisms were not .
	manualset3
163729	7	412220	7	NULL	NULL	0	NULL	FokI polymorphisms 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the BsmI polymorphism is associated with increased risk of T1DM ( BB+B b vs. bb : OR = 1.30 , 95 % CI = 1.03-1 .63 ) , while the FokI , ApaI and TaqI polymorphisms were not .
	manualset3
163730	8	412220	7	NULL	NULL	0	NULL	ApaI polymorphisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the BsmI polymorphism is associated with increased risk of T1DM ( BB+B b vs. bb : OR = 1.30 , 95 % CI = 1.03-1 .63 ) , while the FokI , ApaI and TaqI polymorphisms were not .
	manualset3
163731	9	412220	7	NULL	NULL	0	NULL	TaqI polymorphisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the BsmI polymorphism is associated with increased risk of T1DM ( BB+B b vs. bb : OR = 1.30 , 95 % CI = 1.03-1 .63 ) , while the FokI , ApaI and TaqI polymorphisms were not .
	manualset3
163732	1	412221	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicated that the composition of fibre-like ternary nanoparticles are with atomic ratio of Na : Fe : S = 1 : 1.1 : 1.9 .
	manualset3
163733	2	412221	7	NULL	NULL	NULL	NULL	composition	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicated that the composition of fibre-like ternary nanoparticles are with atomic ratio of Na : Fe : S = 1 : 1.1 : 1.9 .
	manualset3
163734	3	412221	7	NULL	NULL	0	NULL	fibre-like ternary nanoparticles	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the composition of fibre-like ternary nanoparticles are with atomic ratio of Na : Fe : S = 1 : 1.1 : 1.9 .
	manualset3
163735	4	412221	7	NULL	NULL	0	NULL	atomic ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the composition of fibre-like ternary nanoparticles are with atomic ratio of Na : Fe : S = 1 : 1.1 : 1.9 .
	manualset3
163736	5	412221	7	NULL	NULL	0	NULL	Na : Fe : S	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the composition of fibre-like ternary nanoparticles are with atomic ratio of Na : Fe : S = 1 : 1.1 : 1.9 .
	manualset3
163737	6	412221	7	NULL	NULL	0	NULL	1 : 1.1 : 1.9	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the composition of fibre-like ternary nanoparticles are with atomic ratio of Na : Fe : S = 1 : 1.1 : 1.9 .
	manualset3
163738	1	412222	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicated that the level of the dopamine D2 receptor transcript was significantly reduced by SP ( 1-7 ) in nucleus accumbens and frontal cortex but not altered in the striatum .
	manualset3
163739	2	412222	7	NULL	NULL	0	NULL	level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the level of the dopamine D2 receptor transcript was significantly reduced by SP ( 1-7 ) in nucleus accumbens and frontal cortex but not altered in the striatum .
	manualset3
163740	3	412222	7	NULL	NULL	0	NULL	dopamine D2 receptor transcript	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the level of the dopamine D2 receptor transcript was significantly reduced by SP ( 1-7 ) in nucleus accumbens and frontal cortex but not altered in the striatum .
	manualset3
163741	4	412222	7	NULL	NULL	0	NULL	SP ( 1-7 )	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the level of the dopamine D2 receptor transcript was significantly reduced by SP ( 1-7 ) in nucleus accumbens and frontal cortex but not altered in the striatum .
	manualset3
163742	5	412222	7	NULL	NULL	0	NULL	nucleus accumbens	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the level of the dopamine D2 receptor transcript was significantly reduced by SP ( 1-7 ) in nucleus accumbens and frontal cortex but not altered in the striatum .
	manualset3
163743	6	412222	7	NULL	NULL	0	NULL	frontal cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the level of the dopamine D2 receptor transcript was significantly reduced by SP ( 1-7 ) in nucleus accumbens and frontal cortex but not altered in the striatum .
	manualset3
163744	7	412222	7	NULL	NULL	0	NULL	striatum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the level of the dopamine D2 receptor transcript was significantly reduced by SP ( 1-7 ) in nucleus accumbens and frontal cortex but not altered in the striatum .
	manualset3
163745	1	412223	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicated that the minimal amount of template DNA from single blood plasma for accuracy identification was at least about 0.625 ng , the DNA amount extracted from 500 microl of plasma could meet the requirement for PCR amplification .
	manualset3
163746	2	412223	7	NULL	NULL	0	NULL	minimal amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the minimal amount of template DNA from single blood plasma for accuracy identification was at least about 0.625 ng , the DNA amount extracted from 500 microl of plasma could meet the requirement for PCR amplification .
	manualset3
163747	3	412223	7	NULL	NULL	0	NULL	template DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the minimal amount of template DNA from single blood plasma for accuracy identification was at least about 0.625 ng , the DNA amount extracted from 500 microl of plasma could meet the requirement for PCR amplification .
	manualset3
163748	4	412223	7	NULL	NULL	0	NULL	single blood plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the minimal amount of template DNA from single blood plasma for accuracy identification was at least about 0.625 ng , the DNA amount extracted from 500 microl of plasma could meet the requirement for PCR amplification .
	manualset3
163749	5	412223	7	NULL	NULL	0	NULL	 identification 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the minimal amount of template DNA from single blood plasma for accuracy identification was at least about 0.625 ng , the DNA amount extracted from 500 microl of plasma could meet the requirement for PCR amplification .
	manualset3
163750	6	412223	7	NULL	NULL	0	NULL	0.625 ng	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the minimal amount of template DNA from single blood plasma for accuracy identification was at least about 0.625 ng , the DNA amount extracted from 500 microl of plasma could meet the requirement for PCR amplification .
	manualset3
163751	7	412223	7	NULL	NULL	0	NULL	DNA amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the minimal amount of template DNA from single blood plasma for accuracy identification was at least about 0.625 ng , the DNA amount extracted from 500 microl of plasma could meet the requirement for PCR amplification .
	manualset3
163752	8	412223	7	NULL	NULL	0	NULL	500 microl 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the minimal amount of template DNA from single blood plasma for accuracy identification was at least about 0.625 ng , the DNA amount extracted from 500 microl of plasma could meet the requirement for PCR amplification .
	manualset3
163753	9	412223	7	NULL	NULL	0	NULL	plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the minimal amount of template DNA from single blood plasma for accuracy identification was at least about 0.625 ng , the DNA amount extracted from 500 microl of plasma could meet the requirement for PCR amplification .
	manualset3
163754	10	412223	7	NULL	NULL	0	NULL	 requirement	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the minimal amount of template DNA from single blood plasma for accuracy identification was at least about 0.625 ng , the DNA amount extracted from 500 microl of plasma could meet the requirement for PCR amplification .
	manualset3
163755	11	412223	7	NULL	NULL	0	NULL	PCR amplification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the minimal amount of template DNA from single blood plasma for accuracy identification was at least about 0.625 ng , the DNA amount extracted from 500 microl of plasma could meet the requirement for PCR amplification .
	manualset3
163756	1	412224	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicated that the synthesis and release of vWF were increased in the presence of PMA , and secretion of vWF was stimulated by IL-1 .
	manualset3
163757	2	412224	7	NULL	NULL	0	NULL	synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the synthesis and release of vWF were increased in the presence of PMA , and secretion of vWF was stimulated by IL-1 .
	manualset3
163758	3	412224	7	NULL	NULL	0	NULL	release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the synthesis and release of vWF were increased in the presence of PMA , and secretion of vWF was stimulated by IL-1 .
	manualset3
163759	4	412224	7	NULL	NULL	0	NULL	vWF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the synthesis and release of vWF were increased in the presence of PMA , and secretion of vWF was stimulated by IL-1 .
	manualset3
163760	5	412224	7	NULL	NULL	NULL	NULL	presence	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results indicated that the synthesis and release of vWF were increased in the presence of PMA , and secretion of vWF was stimulated by IL-1 .
	manualset3
163761	6	412224	7	NULL	NULL	0	NULL	PMA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the synthesis and release of vWF were increased in the presence of PMA , and secretion of vWF was stimulated by IL-1 .
	manualset3
163762	7	412224	7	NULL	NULL	0	NULL	secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the synthesis and release of vWF were increased in the presence of PMA , and secretion of vWF was stimulated by IL-1 .
	manualset3
163763	8	412224	7	NULL	NULL	0	NULL	vWF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the synthesis and release of vWF were increased in the presence of PMA , and secretion of vWF was stimulated by IL-1 .
	manualset3
163764	9	412224	7	NULL	NULL	0	NULL	IL-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results indicated that the synthesis and release of vWF were increased in the presence of PMA , and secretion of vWF was stimulated by IL-1 .
	manualset3
163765	1	412225	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results infer that 3-phosphoglycerate produced in the chloroplast is not the singular precursor of mitochondrial citrate .
	manualset3
163766	2	412225	7	NULL	NULL	0	NULL	3-phosphoglycerate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The results infer that 3-phosphoglycerate produced in the chloroplast is not the singular precursor of mitochondrial citrate .
	manualset3
163767	3	412225	7	NULL	NULL	0	NULL	chloroplast	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The results infer that 3-phosphoglycerate produced in the chloroplast is not the singular precursor of mitochondrial citrate .
	manualset3
163768	4	412225	7	NULL	NULL	0	NULL	singular precursor 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The results infer that 3-phosphoglycerate produced in the chloroplast is not the singular precursor of mitochondrial citrate .
	manualset3
163769	5	412225	7	NULL	NULL	0	NULL	mitochondrial citrate 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The results infer that 3-phosphoglycerate produced in the chloroplast is not the singular precursor of mitochondrial citrate .
	manualset3
163770	1	412226	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results may be summarized as follows : temporary hemostasis was achieved in 21 patients , bleeding recurred in 8 and 9 patients required emergency surgery .
	manualset3
163771	2	412226	7	NULL	NULL	0	NULL	temporary hemostasis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results may be summarized as follows : temporary hemostasis was achieved in 21 patients , bleeding recurred in 8 and 9 patients required emergency surgery .
	manualset3
163772	3	412226	7	NULL	NULL	0	NULL	 21 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results may be summarized as follows : temporary hemostasis was achieved in 21 patients , bleeding recurred in 8 and 9 patients required emergency surgery .
	manualset3
163773	4	412226	7	NULL	NULL	0	NULL	bleeding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results may be summarized as follows : temporary hemostasis was achieved in 21 patients , bleeding recurred in 8 and 9 patients required emergency surgery .
	manualset3
163774	5	412226	7	NULL	NULL	0	NULL	8 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results may be summarized as follows : temporary hemostasis was achieved in 21 patients , bleeding recurred in 8 and 9 patients required emergency surgery .
	manualset3
163775	6	412226	7	NULL	NULL	0	NULL	9 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results may be summarized as follows : temporary hemostasis was achieved in 21 patients , bleeding recurred in 8 and 9 patients required emergency surgery .
	manualset3
163776	7	412226	7	NULL	NULL	0	NULL	emergency surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results may be summarized as follows : temporary hemostasis was achieved in 21 patients , bleeding recurred in 8 and 9 patients required emergency surgery .
	manualset3
163777	1	412227	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results obtained are now used as a benchmark in the participating facilities and can be used by others to gauge the effectiveness of care .
	manualset3
163778	2	412227	7	NULL	NULL	0	NULL	facilities	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained are now used as a benchmark in the participating facilities and can be used by others to gauge the effectiveness of care .
	manualset3
163779	3	412227	7	NULL	NULL	NULL	NULL	effectiveness	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results obtained are now used as a benchmark in the participating facilities and can be used by others to gauge the effectiveness of care .
	manualset3
163780	4	412227	7	NULL	NULL	0	NULL	care	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained are now used as a benchmark in the participating facilities and can be used by others to gauge the effectiveness of care .
	manualset3
163781	1	412228	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results obtained corresponded to the features of habituation in other sensory systems .
	manualset3
163782	2	412228	7	NULL	NULL	NULL	NULL	habituation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results obtained corresponded to the features of habituation in other sensory systems .
	manualset3
163783	3	412228	7	NULL	NULL	0	NULL	sensory systems	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained corresponded to the features of habituation in other sensory systems .
	manualset3
163784	1	412229	7	NULL	NULL	0	NULL	Ac-Thr-Ile-Nle-Nle-Gln-Arg-NH2	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Ac-Thr-Ile-Nle-Nle-Gln-Arg-NH2 , incorporation of 2-aminobenzoic acid in place of the acetyl group as the donor and p-NO2-Phe at the P1 ' position as acceptor gave the intramolecularly quenched fluorogenic substrate .
	manualset3
163785	2	412229	7	NULL	NULL	0	NULL	2-aminobenzoic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ac-Thr-Ile-Nle-Nle-Gln-Arg-NH2 , incorporation of 2-aminobenzoic acid in place of the acetyl group as the donor and p-NO2-Phe at the P1 ' position as acceptor gave the intramolecularly quenched fluorogenic substrate .
	manualset3
163786	3	412229	7	NULL	NULL	0	NULL	 acetyl group	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ac-Thr-Ile-Nle-Nle-Gln-Arg-NH2 , incorporation of 2-aminobenzoic acid in place of the acetyl group as the donor and p-NO2-Phe at the P1 ' position as acceptor gave the intramolecularly quenched fluorogenic substrate .
	manualset3
163787	4	412229	7	NULL	NULL	0	NULL	donor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ac-Thr-Ile-Nle-Nle-Gln-Arg-NH2 , incorporation of 2-aminobenzoic acid in place of the acetyl group as the donor and p-NO2-Phe at the P1 ' position as acceptor gave the intramolecularly quenched fluorogenic substrate .
	manualset3
163788	5	412229	7	NULL	NULL	0	NULL	 p-NO2-Phe	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ac-Thr-Ile-Nle-Nle-Gln-Arg-NH2 , incorporation of 2-aminobenzoic acid in place of the acetyl group as the donor and p-NO2-Phe at the P1 ' position as acceptor gave the intramolecularly quenched fluorogenic substrate .
	manualset3
163789	6	412229	7	NULL	NULL	0	NULL	P1 ' position	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ac-Thr-Ile-Nle-Nle-Gln-Arg-NH2 , incorporation of 2-aminobenzoic acid in place of the acetyl group as the donor and p-NO2-Phe at the P1 ' position as acceptor gave the intramolecularly quenched fluorogenic substrate .
	manualset3
163790	7	412229	7	NULL	NULL	0	NULL	acceptor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ac-Thr-Ile-Nle-Nle-Gln-Arg-NH2 , incorporation of 2-aminobenzoic acid in place of the acetyl group as the donor and p-NO2-Phe at the P1 ' position as acceptor gave the intramolecularly quenched fluorogenic substrate .
	manualset3
163791	8	412229	7	NULL	NULL	0	NULL	fluorogenic substrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ac-Thr-Ile-Nle-Nle-Gln-Arg-NH2 , incorporation of 2-aminobenzoic acid in place of the acetyl group as the donor and p-NO2-Phe at the P1 ' position as acceptor gave the intramolecularly quenched fluorogenic substrate .
	manualset3
163792	1	412230	7	NULL	NULL	NULL	NULL	 results 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results obtained in the present work will strengthen the development of biotechnology programs to improve the productive potential and conservation of the collared peccary .
	manualset3
163793	2	412230	7	NULL	NULL	NULL	NULL	present work	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results obtained in the present work will strengthen the development of biotechnology programs to improve the productive potential and conservation of the collared peccary .
	manualset3
163794	3	412230	7	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained in the present work will strengthen the development of biotechnology programs to improve the productive potential and conservation of the collared peccary .
	manualset3
163795	4	412230	7	NULL	NULL	0	NULL	biotechnology programs	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained in the present work will strengthen the development of biotechnology programs to improve the productive potential and conservation of the collared peccary .
	manualset3
163796	5	412230	7	NULL	NULL	0	NULL	productive potential 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained in the present work will strengthen the development of biotechnology programs to improve the productive potential and conservation of the collared peccary .
	manualset3
163797	6	412230	7	NULL	NULL	0	NULL	conservation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained in the present work will strengthen the development of biotechnology programs to improve the productive potential and conservation of the collared peccary .
	manualset3
163798	7	412230	7	NULL	NULL	0	NULL	collared peccary	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained in the present work will strengthen the development of biotechnology programs to improve the productive potential and conservation of the collared peccary .
	manualset3
163810	1	412231	7	NULL	NULL	NULL	NULL	 results 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results obtained in this work indicate that the fragmentation behavior of colloidal aggregates depends on their fractal structure .
	manualset3
163811	2	412231	7	NULL	NULL	0	NULL	work	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained in this work indicate that the fragmentation behavior of colloidal aggregates depends on their fractal structure .
	manualset3
163812	3	412231	7	NULL	NULL	0	NULL	fragmentation behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained in this work indicate that the fragmentation behavior of colloidal aggregates depends on their fractal structure .
	manualset3
163813	4	412231	7	NULL	NULL	0	NULL	colloidal aggregates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained in this work indicate that the fragmentation behavior of colloidal aggregates depends on their fractal structure .
	manualset3
163814	5	412231	7	NULL	NULL	0	NULL	 fractal structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained in this work indicate that the fragmentation behavior of colloidal aggregates depends on their fractal structure .
	manualset3
163815	1	412232	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results obtained indicate a highly significant increase in prolactinemia after 60 minutes in a patient undergoing chronic L-Dopa + benserazide therapy , compared to both healthy subjects and patients receiving other drugs .
	manualset3
163816	2	412232	7	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained indicate a highly significant increase in prolactinemia after 60 minutes in a patient undergoing chronic L-Dopa + benserazide therapy , compared to both healthy subjects and patients receiving other drugs .
	manualset3
163817	3	412232	7	NULL	NULL	0	NULL	prolactinemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained indicate a highly significant increase in prolactinemia after 60 minutes in a patient undergoing chronic L-Dopa + benserazide therapy , compared to both healthy subjects and patients receiving other drugs .
	manualset3
163818	4	412232	7	NULL	NULL	0	NULL	60 minutes	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained indicate a highly significant increase in prolactinemia after 60 minutes in a patient undergoing chronic L-Dopa + benserazide therapy , compared to both healthy subjects and patients receiving other drugs .
	manualset3
163819	5	412232	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained indicate a highly significant increase in prolactinemia after 60 minutes in a patient undergoing chronic L-Dopa + benserazide therapy , compared to both healthy subjects and patients receiving other drugs .
	manualset3
163820	6	412232	7	NULL	NULL	0	NULL	chronic L-Dopa + benserazide therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained indicate a highly significant increase in prolactinemia after 60 minutes in a patient undergoing chronic L-Dopa + benserazide therapy , compared to both healthy subjects and patients receiving other drugs .
	manualset3
163821	7	412232	7	NULL	NULL	0	NULL	healthy subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained indicate a highly significant increase in prolactinemia after 60 minutes in a patient undergoing chronic L-Dopa + benserazide therapy , compared to both healthy subjects and patients receiving other drugs .
	manualset3
163822	8	412232	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained indicate a highly significant increase in prolactinemia after 60 minutes in a patient undergoing chronic L-Dopa + benserazide therapy , compared to both healthy subjects and patients receiving other drugs .
	manualset3
163823	9	412232	7	NULL	NULL	0	NULL	drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained indicate a highly significant increase in prolactinemia after 60 minutes in a patient undergoing chronic L-Dopa + benserazide therapy , compared to both healthy subjects and patients receiving other drugs .
	manualset3
163824	1	412233	7	NULL	NULL	NULL	NULL	results 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results obtained indicate that the presence of the `` L '' insert affects several biochemical properties of CK1alpha : ( a ) it increases the apparent Km for ATP twofold , from approximately 30 to approximately 60 microM ; ( b ) it decreases the sensitivity to the CKI-7 inhibitor , raising the I50 values from 113 to approximately 230 microM ; ( c ) it greatly decreases the heat stability of the enzyme at 40 degrees C. In addition , the insertion of the `` L '' fragment exerts very important effects on some cellular properties of the enzyme .
	manualset3
163825	2	412233	7	NULL	NULL	NULL	NULL	presence	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results obtained indicate that the presence of the `` L '' insert affects several biochemical properties of CK1alpha : ( a ) it increases the apparent Km for ATP twofold , from approximately 30 to approximately 60 microM ; ( b ) it decreases the sensitivity to the CKI-7 inhibitor , raising the I50 values from 113 to approximately 230 microM ; ( c ) it greatly decreases the heat stability of the enzyme at 40 degrees C. In addition , the insertion of the `` L '' fragment exerts very important effects on some cellular properties of the enzyme .
	manualset3
163826	3	412233	7	NULL	NULL	0	NULL	`` L '' insert 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained indicate that the presence of the `` L '' insert affects several biochemical properties of CK1alpha : ( a ) it increases the apparent Km for ATP twofold , from approximately 30 to approximately 60 microM ; ( b ) it decreases the sensitivity to the CKI-7 inhibitor , raising the I50 values from 113 to approximately 230 microM ; ( c ) it greatly decreases the heat stability of the enzyme at 40 degrees C. In addition , the insertion of the `` L '' fragment exerts very important effects on some cellular properties of the enzyme .
	manualset3
163827	4	412233	7	NULL	NULL	0	NULL	biochemical properties 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained indicate that the presence of the `` L '' insert affects several biochemical properties of CK1alpha : ( a ) it increases the apparent Km for ATP twofold , from approximately 30 to approximately 60 microM ; ( b ) it decreases the sensitivity to the CKI-7 inhibitor , raising the I50 values from 113 to approximately 230 microM ; ( c ) it greatly decreases the heat stability of the enzyme at 40 degrees C. In addition , the insertion of the `` L '' fragment exerts very important effects on some cellular properties of the enzyme .
	manualset3
163828	5	412233	7	NULL	NULL	0	NULL	CK1alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained indicate that the presence of the `` L '' insert affects several biochemical properties of CK1alpha : ( a ) it increases the apparent Km for ATP twofold , from approximately 30 to approximately 60 microM ; ( b ) it decreases the sensitivity to the CKI-7 inhibitor , raising the I50 values from 113 to approximately 230 microM ; ( c ) it greatly decreases the heat stability of the enzyme at 40 degrees C. In addition , the insertion of the `` L '' fragment exerts very important effects on some cellular properties of the enzyme .
	manualset3
163829	6	412233	7	NULL	NULL	0	NULL	apparent Km	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained indicate that the presence of the `` L '' insert affects several biochemical properties of CK1alpha : ( a ) it increases the apparent Km for ATP twofold , from approximately 30 to approximately 60 microM ; ( b ) it decreases the sensitivity to the CKI-7 inhibitor , raising the I50 values from 113 to approximately 230 microM ; ( c ) it greatly decreases the heat stability of the enzyme at 40 degrees C. In addition , the insertion of the `` L '' fragment exerts very important effects on some cellular properties of the enzyme .
	manualset3
163830	7	412233	7	NULL	NULL	0	NULL	ATP 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained indicate that the presence of the `` L '' insert affects several biochemical properties of CK1alpha : ( a ) it increases the apparent Km for ATP twofold , from approximately 30 to approximately 60 microM ; ( b ) it decreases the sensitivity to the CKI-7 inhibitor , raising the I50 values from 113 to approximately 230 microM ; ( c ) it greatly decreases the heat stability of the enzyme at 40 degrees C. In addition , the insertion of the `` L '' fragment exerts very important effects on some cellular properties of the enzyme .
	manualset3
163831	8	412233	7	NULL	NULL	0	NULL	twofold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained indicate that the presence of the `` L '' insert affects several biochemical properties of CK1alpha : ( a ) it increases the apparent Km for ATP twofold , from approximately 30 to approximately 60 microM ; ( b ) it decreases the sensitivity to the CKI-7 inhibitor , raising the I50 values from 113 to approximately 230 microM ; ( c ) it greatly decreases the heat stability of the enzyme at 40 degrees C. In addition , the insertion of the `` L '' fragment exerts very important effects on some cellular properties of the enzyme .
	manualset3
163832	9	412233	7	NULL	NULL	0	NULL	30 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained indicate that the presence of the `` L '' insert affects several biochemical properties of CK1alpha : ( a ) it increases the apparent Km for ATP twofold , from approximately 30 to approximately 60 microM ; ( b ) it decreases the sensitivity to the CKI-7 inhibitor , raising the I50 values from 113 to approximately 230 microM ; ( c ) it greatly decreases the heat stability of the enzyme at 40 degrees C. In addition , the insertion of the `` L '' fragment exerts very important effects on some cellular properties of the enzyme .
	manualset3
163833	10	412233	7	NULL	NULL	0	NULL	60 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained indicate that the presence of the `` L '' insert affects several biochemical properties of CK1alpha : ( a ) it increases the apparent Km for ATP twofold , from approximately 30 to approximately 60 microM ; ( b ) it decreases the sensitivity to the CKI-7 inhibitor , raising the I50 values from 113 to approximately 230 microM ; ( c ) it greatly decreases the heat stability of the enzyme at 40 degrees C. In addition , the insertion of the `` L '' fragment exerts very important effects on some cellular properties of the enzyme .
	manualset3
163834	11	412233	7	NULL	NULL	0	NULL	sensitivity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained indicate that the presence of the `` L '' insert affects several biochemical properties of CK1alpha : ( a ) it increases the apparent Km for ATP twofold , from approximately 30 to approximately 60 microM ; ( b ) it decreases the sensitivity to the CKI-7 inhibitor , raising the I50 values from 113 to approximately 230 microM ; ( c ) it greatly decreases the heat stability of the enzyme at 40 degrees C. In addition , the insertion of the `` L '' fragment exerts very important effects on some cellular properties of the enzyme .
	manualset3
163835	12	412233	7	NULL	NULL	0	NULL	CKI-7 inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained indicate that the presence of the `` L '' insert affects several biochemical properties of CK1alpha : ( a ) it increases the apparent Km for ATP twofold , from approximately 30 to approximately 60 microM ; ( b ) it decreases the sensitivity to the CKI-7 inhibitor , raising the I50 values from 113 to approximately 230 microM ; ( c ) it greatly decreases the heat stability of the enzyme at 40 degrees C. In addition , the insertion of the `` L '' fragment exerts very important effects on some cellular properties of the enzyme .
	manualset3
163836	13	412233	7	NULL	NULL	0	NULL	I50 values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained indicate that the presence of the `` L '' insert affects several biochemical properties of CK1alpha : ( a ) it increases the apparent Km for ATP twofold , from approximately 30 to approximately 60 microM ; ( b ) it decreases the sensitivity to the CKI-7 inhibitor , raising the I50 values from 113 to approximately 230 microM ; ( c ) it greatly decreases the heat stability of the enzyme at 40 degrees C. In addition , the insertion of the `` L '' fragment exerts very important effects on some cellular properties of the enzyme .
	manualset3
163837	14	412233	7	NULL	NULL	0	NULL	113 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained indicate that the presence of the `` L '' insert affects several biochemical properties of CK1alpha : ( a ) it increases the apparent Km for ATP twofold , from approximately 30 to approximately 60 microM ; ( b ) it decreases the sensitivity to the CKI-7 inhibitor , raising the I50 values from 113 to approximately 230 microM ; ( c ) it greatly decreases the heat stability of the enzyme at 40 degrees C. In addition , the insertion of the `` L '' fragment exerts very important effects on some cellular properties of the enzyme .
	manualset3
163838	15	412233	7	NULL	NULL	0	NULL	230 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained indicate that the presence of the `` L '' insert affects several biochemical properties of CK1alpha : ( a ) it increases the apparent Km for ATP twofold , from approximately 30 to approximately 60 microM ; ( b ) it decreases the sensitivity to the CKI-7 inhibitor , raising the I50 values from 113 to approximately 230 microM ; ( c ) it greatly decreases the heat stability of the enzyme at 40 degrees C. In addition , the insertion of the `` L '' fragment exerts very important effects on some cellular properties of the enzyme .
	manualset3
163839	16	412233	7	NULL	NULL	0	NULL	heat stability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained indicate that the presence of the `` L '' insert affects several biochemical properties of CK1alpha : ( a ) it increases the apparent Km for ATP twofold , from approximately 30 to approximately 60 microM ; ( b ) it decreases the sensitivity to the CKI-7 inhibitor , raising the I50 values from 113 to approximately 230 microM ; ( c ) it greatly decreases the heat stability of the enzyme at 40 degrees C. In addition , the insertion of the `` L '' fragment exerts very important effects on some cellular properties of the enzyme .
	manualset3
163840	17	412233	7	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained indicate that the presence of the `` L '' insert affects several biochemical properties of CK1alpha : ( a ) it increases the apparent Km for ATP twofold , from approximately 30 to approximately 60 microM ; ( b ) it decreases the sensitivity to the CKI-7 inhibitor , raising the I50 values from 113 to approximately 230 microM ; ( c ) it greatly decreases the heat stability of the enzyme at 40 degrees C. In addition , the insertion of the `` L '' fragment exerts very important effects on some cellular properties of the enzyme .
	manualset3
163841	18	412233	7	NULL	NULL	0	NULL	40 degrees C	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained indicate that the presence of the `` L '' insert affects several biochemical properties of CK1alpha : ( a ) it increases the apparent Km for ATP twofold , from approximately 30 to approximately 60 microM ; ( b ) it decreases the sensitivity to the CKI-7 inhibitor , raising the I50 values from 113 to approximately 230 microM ; ( c ) it greatly decreases the heat stability of the enzyme at 40 degrees C. In addition , the insertion of the `` L '' fragment exerts very important effects on some cellular properties of the enzyme .
	manualset3
163842	19	412233	7	NULL	NULL	0	NULL	 addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained indicate that the presence of the `` L '' insert affects several biochemical properties of CK1alpha : ( a ) it increases the apparent Km for ATP twofold , from approximately 30 to approximately 60 microM ; ( b ) it decreases the sensitivity to the CKI-7 inhibitor , raising the I50 values from 113 to approximately 230 microM ; ( c ) it greatly decreases the heat stability of the enzyme at 40 degrees C. In addition , the insertion of the `` L '' fragment exerts very important effects on some cellular properties of the enzyme .
	manualset3
163843	20	412233	7	NULL	NULL	0	NULL	insertion 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained indicate that the presence of the `` L '' insert affects several biochemical properties of CK1alpha : ( a ) it increases the apparent Km for ATP twofold , from approximately 30 to approximately 60 microM ; ( b ) it decreases the sensitivity to the CKI-7 inhibitor , raising the I50 values from 113 to approximately 230 microM ; ( c ) it greatly decreases the heat stability of the enzyme at 40 degrees C. In addition , the insertion of the `` L '' fragment exerts very important effects on some cellular properties of the enzyme .
	manualset3
163844	21	412233	7	NULL	NULL	0	NULL	`` L '' fragment 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained indicate that the presence of the `` L '' insert affects several biochemical properties of CK1alpha : ( a ) it increases the apparent Km for ATP twofold , from approximately 30 to approximately 60 microM ; ( b ) it decreases the sensitivity to the CKI-7 inhibitor , raising the I50 values from 113 to approximately 230 microM ; ( c ) it greatly decreases the heat stability of the enzyme at 40 degrees C. In addition , the insertion of the `` L '' fragment exerts very important effects on some cellular properties of the enzyme .
	manualset3
163845	22	412233	7	NULL	NULL	0	NULL	cellular properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained indicate that the presence of the `` L '' insert affects several biochemical properties of CK1alpha : ( a ) it increases the apparent Km for ATP twofold , from approximately 30 to approximately 60 microM ; ( b ) it decreases the sensitivity to the CKI-7 inhibitor , raising the I50 values from 113 to approximately 230 microM ; ( c ) it greatly decreases the heat stability of the enzyme at 40 degrees C. In addition , the insertion of the `` L '' fragment exerts very important effects on some cellular properties of the enzyme .
	manualset3
163846	23	412233	7	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained indicate that the presence of the `` L '' insert affects several biochemical properties of CK1alpha : ( a ) it increases the apparent Km for ATP twofold , from approximately 30 to approximately 60 microM ; ( b ) it decreases the sensitivity to the CKI-7 inhibitor , raising the I50 values from 113 to approximately 230 microM ; ( c ) it greatly decreases the heat stability of the enzyme at 40 degrees C. In addition , the insertion of the `` L '' fragment exerts very important effects on some cellular properties of the enzyme .
	manualset3
163847	1	412234	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results obtained show that in this loading situation the maximum stress values ( both for tension and compression ) are in the area just below the subtrochanteric zone ; while going up along the borders of the diaphysis , the tension trends do not vary appreciably .
	manualset3
163848	2	412234	7	NULL	NULL	0	NULL	situation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained show that in this loading situation the maximum stress values ( both for tension and compression ) are in the area just below the subtrochanteric zone ; while going up along the borders of the diaphysis , the tension trends do not vary appreciably .
	manualset3
163849	3	412234	7	NULL	NULL	0	NULL	maximum stress values 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained show that in this loading situation the maximum stress values ( both for tension and compression ) are in the area just below the subtrochanteric zone ; while going up along the borders of the diaphysis , the tension trends do not vary appreciably .
	manualset3
163850	4	412234	7	NULL	NULL	NULL	NULL	tension	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results obtained show that in this loading situation the maximum stress values ( both for tension and compression ) are in the area just below the subtrochanteric zone ; while going up along the borders of the diaphysis , the tension trends do not vary appreciably .
	manualset3
163851	5	412234	7	NULL	NULL	NULL	NULL	compression	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results obtained show that in this loading situation the maximum stress values ( both for tension and compression ) are in the area just below the subtrochanteric zone ; while going up along the borders of the diaphysis , the tension trends do not vary appreciably .
	manualset3
163852	6	412234	7	NULL	NULL	0	NULL	area	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained show that in this loading situation the maximum stress values ( both for tension and compression ) are in the area just below the subtrochanteric zone ; while going up along the borders of the diaphysis , the tension trends do not vary appreciably .
	manualset3
163853	7	412234	7	NULL	NULL	0	NULL	subtrochanteric zone	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained show that in this loading situation the maximum stress values ( both for tension and compression ) are in the area just below the subtrochanteric zone ; while going up along the borders of the diaphysis , the tension trends do not vary appreciably .
	manualset3
163854	8	412234	7	NULL	NULL	0	NULL	borders	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained show that in this loading situation the maximum stress values ( both for tension and compression ) are in the area just below the subtrochanteric zone ; while going up along the borders of the diaphysis , the tension trends do not vary appreciably .
	manualset3
163855	9	412234	7	NULL	NULL	0	NULL	diaphysis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained show that in this loading situation the maximum stress values ( both for tension and compression ) are in the area just below the subtrochanteric zone ; while going up along the borders of the diaphysis , the tension trends do not vary appreciably .
	manualset3
163856	10	412234	7	NULL	NULL	0	NULL	 tension	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained show that in this loading situation the maximum stress values ( both for tension and compression ) are in the area just below the subtrochanteric zone ; while going up along the borders of the diaphysis , the tension trends do not vary appreciably .
	manualset3
163857	1	412235	7	NULL	NULL	0	NULL	FDG-PET	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of FDG-PET and CT were compared with the surgical and pathologic results .
	manualset3
163858	2	412235	7	NULL	NULL	0	NULL	 CT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of FDG-PET and CT were compared with the surgical and pathologic results .
	manualset3
163859	3	412235	7	NULL	NULL	0	NULL	 surgical result	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of FDG-PET and CT were compared with the surgical and pathologic results .
	manualset3
163860	4	412235	7	NULL	NULL	0	NULL	pathologic results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of FDG-PET and CT were compared with the surgical and pathologic results .
	manualset3
163861	5	412235	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of FDG-PET and CT were compared with the surgical and pathologic results .
	manualset3
163862	1	412236	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of Monte Carlo simulations indicate that effective glutaraldehyde concentrations can be maintained for the duration of a vessel 's oceanic transit ( approximately 9-12 days ) : During this transit , glutaraldehyde concentrations were predicted to decrease by approximately 10 % from initial treatment levels ( e.g. , 500 mgL ( -1 ) ) .
	manualset3
163863	2	412236	7	NULL	NULL	0	NULL	Monte Carlo simulations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of Monte Carlo simulations indicate that effective glutaraldehyde concentrations can be maintained for the duration of a vessel 's oceanic transit ( approximately 9-12 days ) : During this transit , glutaraldehyde concentrations were predicted to decrease by approximately 10 % from initial treatment levels ( e.g. , 500 mgL ( -1 ) ) .
	manualset3
163864	3	412236	7	NULL	NULL	0	NULL	 glutaraldehyde	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of Monte Carlo simulations indicate that effective glutaraldehyde concentrations can be maintained for the duration of a vessel 's oceanic transit ( approximately 9-12 days ) : During this transit , glutaraldehyde concentrations were predicted to decrease by approximately 10 % from initial treatment levels ( e.g. , 500 mgL ( -1 ) ) .
	manualset3
163865	4	412236	7	NULL	NULL	0	NULL	concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of Monte Carlo simulations indicate that effective glutaraldehyde concentrations can be maintained for the duration of a vessel 's oceanic transit ( approximately 9-12 days ) : During this transit , glutaraldehyde concentrations were predicted to decrease by approximately 10 % from initial treatment levels ( e.g. , 500 mgL ( -1 ) ) .
	manualset3
163866	5	412236	7	NULL	NULL	0	NULL	duration 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of Monte Carlo simulations indicate that effective glutaraldehyde concentrations can be maintained for the duration of a vessel 's oceanic transit ( approximately 9-12 days ) : During this transit , glutaraldehyde concentrations were predicted to decrease by approximately 10 % from initial treatment levels ( e.g. , 500 mgL ( -1 ) ) .
	manualset3
163867	6	412236	7	NULL	NULL	0	NULL	vessel 's oceanic transit	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of Monte Carlo simulations indicate that effective glutaraldehyde concentrations can be maintained for the duration of a vessel 's oceanic transit ( approximately 9-12 days ) : During this transit , glutaraldehyde concentrations were predicted to decrease by approximately 10 % from initial treatment levels ( e.g. , 500 mgL ( -1 ) ) .
	manualset3
163868	7	412236	7	NULL	NULL	0	NULL	 9-12 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of Monte Carlo simulations indicate that effective glutaraldehyde concentrations can be maintained for the duration of a vessel 's oceanic transit ( approximately 9-12 days ) : During this transit , glutaraldehyde concentrations were predicted to decrease by approximately 10 % from initial treatment levels ( e.g. , 500 mgL ( -1 ) ) .
	manualset3
163869	8	412236	7	NULL	NULL	0	NULL	transit	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of Monte Carlo simulations indicate that effective glutaraldehyde concentrations can be maintained for the duration of a vessel 's oceanic transit ( approximately 9-12 days ) : During this transit , glutaraldehyde concentrations were predicted to decrease by approximately 10 % from initial treatment levels ( e.g. , 500 mgL ( -1 ) ) .
	manualset3
163870	9	412236	7	NULL	NULL	0	NULL	glutaraldehyde	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of Monte Carlo simulations indicate that effective glutaraldehyde concentrations can be maintained for the duration of a vessel 's oceanic transit ( approximately 9-12 days ) : During this transit , glutaraldehyde concentrations were predicted to decrease by approximately 10 % from initial treatment levels ( e.g. , 500 mgL ( -1 ) ) .
	manualset3
163871	10	412236	7	NULL	NULL	0	NULL	concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of Monte Carlo simulations indicate that effective glutaraldehyde concentrations can be maintained for the duration of a vessel 's oceanic transit ( approximately 9-12 days ) : During this transit , glutaraldehyde concentrations were predicted to decrease by approximately 10 % from initial treatment levels ( e.g. , 500 mgL ( -1 ) ) .
	manualset3
163872	11	412236	7	NULL	NULL	0	NULL	 10 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of Monte Carlo simulations indicate that effective glutaraldehyde concentrations can be maintained for the duration of a vessel 's oceanic transit ( approximately 9-12 days ) : During this transit , glutaraldehyde concentrations were predicted to decrease by approximately 10 % from initial treatment levels ( e.g. , 500 mgL ( -1 ) ) .
	manualset3
163873	12	412236	7	NULL	NULL	0	NULL	initial treatment levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of Monte Carlo simulations indicate that effective glutaraldehyde concentrations can be maintained for the duration of a vessel 's oceanic transit ( approximately 9-12 days ) : During this transit , glutaraldehyde concentrations were predicted to decrease by approximately 10 % from initial treatment levels ( e.g. , 500 mgL ( -1 ) ) .
	manualset3
163874	13	412236	7	NULL	NULL	0	NULL	500 mgL ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of Monte Carlo simulations indicate that effective glutaraldehyde concentrations can be maintained for the duration of a vessel 's oceanic transit ( approximately 9-12 days ) : During this transit , glutaraldehyde concentrations were predicted to decrease by approximately 10 % from initial treatment levels ( e.g. , 500 mgL ( -1 ) ) .
	manualset3
163875	1	412237	7	NULL	NULL	0	NULL	Academic achievement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Academic achievement among undergraduate nursing students : the development and test of a causal model .
	manualset3
163876	2	412237	7	NULL	NULL	NULL	NULL	undergraduate  nursing students	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Academic achievement among undergraduate nursing students : the development and test of a causal model .
	manualset3
163878	4	412237	7	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Academic achievement among undergraduate nursing students : the development and test of a causal model .
	manualset3
163879	5	412237	7	NULL	NULL	0	NULL	test 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Academic achievement among undergraduate nursing students : the development and test of a causal model .
	manualset3
163880	6	412237	7	NULL	NULL	NULL	NULL	causal model	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Academic achievement among undergraduate nursing students : the development and test of a causal model .
	manualset3
163881	1	412238	7	NULL	NULL	0	NULL	 results	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of X-ray diffraction indicated that nitrendipine in microspheres was disordered , suggesting that nitrendipine was highly dispersed in microspheres .
	manualset3
163882	2	412238	7	NULL	NULL	0	NULL	X-ray diffraction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of X-ray diffraction indicated that nitrendipine in microspheres was disordered , suggesting that nitrendipine was highly dispersed in microspheres .
	manualset3
163883	3	412238	7	NULL	NULL	NULL	NULL	nitrendipine	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of X-ray diffraction indicated that nitrendipine in microspheres was disordered , suggesting that nitrendipine was highly dispersed in microspheres .
	manualset3
163884	4	412238	7	NULL	NULL	0	NULL	microspheres	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of X-ray diffraction indicated that nitrendipine in microspheres was disordered , suggesting that nitrendipine was highly dispersed in microspheres .
	manualset3
163885	5	412238	7	NULL	NULL	0	NULL	nitrendipine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of X-ray diffraction indicated that nitrendipine in microspheres was disordered , suggesting that nitrendipine was highly dispersed in microspheres .
	manualset3
163886	6	412238	7	NULL	NULL	0	NULL	microspheres 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of X-ray diffraction indicated that nitrendipine in microspheres was disordered , suggesting that nitrendipine was highly dispersed in microspheres .
	manualset3
163887	1	412239	7	NULL	NULL	0	NULL	 results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of amblyopia therapy depend on the degree of anisometropia , the co-existence of strabismus , the compliance with penalization , and the presence of retinal abnormalities .
	manualset3
163888	2	412239	7	NULL	NULL	0	NULL	amblyopia therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of amblyopia therapy depend on the degree of anisometropia , the co-existence of strabismus , the compliance with penalization , and the presence of retinal abnormalities .
	manualset3
163889	3	412239	7	NULL	NULL	0	NULL	 degree	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of amblyopia therapy depend on the degree of anisometropia , the co-existence of strabismus , the compliance with penalization , and the presence of retinal abnormalities .
	manualset3
163890	4	412239	7	NULL	NULL	0	NULL	anisometropia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of amblyopia therapy depend on the degree of anisometropia , the co-existence of strabismus , the compliance with penalization , and the presence of retinal abnormalities .
	manualset3
163891	5	412239	7	NULL	NULL	0	NULL	co-existence	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of amblyopia therapy depend on the degree of anisometropia , the co-existence of strabismus , the compliance with penalization , and the presence of retinal abnormalities .
	manualset3
163892	6	412239	7	NULL	NULL	0	NULL	strabismus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of amblyopia therapy depend on the degree of anisometropia , the co-existence of strabismus , the compliance with penalization , and the presence of retinal abnormalities .
	manualset3
163893	7	412239	7	NULL	NULL	0	NULL	compliance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of amblyopia therapy depend on the degree of anisometropia , the co-existence of strabismus , the compliance with penalization , and the presence of retinal abnormalities .
	manualset3
163894	8	412239	7	NULL	NULL	0	NULL	penalization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of amblyopia therapy depend on the degree of anisometropia , the co-existence of strabismus , the compliance with penalization , and the presence of retinal abnormalities .
	manualset3
163895	9	412239	7	NULL	NULL	0	NULL	 presence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of amblyopia therapy depend on the degree of anisometropia , the co-existence of strabismus , the compliance with penalization , and the presence of retinal abnormalities .
	manualset3
163896	10	412239	7	NULL	NULL	0	NULL	 retinal abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of amblyopia therapy depend on the degree of anisometropia , the co-existence of strabismus , the compliance with penalization , and the presence of retinal abnormalities .
	manualset3
163897	1	412240	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of excision of the trapezium .
	manualset3
163898	2	412240	7	NULL	NULL	0	NULL	 excision	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of excision of the trapezium .
	manualset3
163899	3	412240	7	NULL	NULL	0	NULL	 trapezium	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of excision of the trapezium .
	manualset3
163900	1	412241	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of methylation analysis have raised the possibility that this release is in part due to cleavage of the chitobiosyl core .
	manualset3
163901	2	412241	7	NULL	NULL	NULL	NULL	methylation analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of methylation analysis have raised the possibility that this release is in part due to cleavage of the chitobiosyl core .
	manualset3
163903	4	412241	7	NULL	NULL	0	NULL	possibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of methylation analysis have raised the possibility that this release is in part due to cleavage of the chitobiosyl core .
	manualset3
163904	5	412241	7	NULL	NULL	0	NULL	release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of methylation analysis have raised the possibility that this release is in part due to cleavage of the chitobiosyl core .
	manualset3
163905	6	412241	7	NULL	NULL	0	NULL	cleavage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of methylation analysis have raised the possibility that this release is in part due to cleavage of the chitobiosyl core .
	manualset3
163906	7	412241	7	NULL	NULL	0	NULL	chitobiosyl core	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of methylation analysis have raised the possibility that this release is in part due to cleavage of the chitobiosyl core .
	manualset3
163907	1	412242	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of our study suggest a small but replicable context-dependent influence of the APOA5 gene region on plasma TG levels in young , healthy individuals .
	manualset3
163908	2	412242	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of our study suggest a small but replicable context-dependent influence of the APOA5 gene region on plasma TG levels in young , healthy individuals .
	manualset3
163909	3	412242	7	NULL	NULL	0	NULL	small 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of our study suggest a small but replicable context-dependent influence of the APOA5 gene region on plasma TG levels in young , healthy individuals .
	manualset3
163910	4	412242	7	NULL	NULL	0	NULL	context-dependent influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of our study suggest a small but replicable context-dependent influence of the APOA5 gene region on plasma TG levels in young , healthy individuals .
	manualset3
163911	5	412242	7	NULL	NULL	0	NULL	APOA5 gene region	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of our study suggest a small but replicable context-dependent influence of the APOA5 gene region on plasma TG levels in young , healthy individuals .
	manualset3
163912	6	412242	7	NULL	NULL	0	NULL	plasma TG levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of our study suggest a small but replicable context-dependent influence of the APOA5 gene region on plasma TG levels in young , healthy individuals .
	manualset3
163913	7	412242	7	NULL	NULL	0	NULL	 healthy individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of our study suggest a small but replicable context-dependent influence of the APOA5 gene region on plasma TG levels in young , healthy individuals .
	manualset3
163914	1	412243	7	NULL	NULL	NULL	NULL	Clinico-dynamic aspects	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Clinico-dynamic aspects of long-term remissions in schizophrenia ) .
	manualset3
163915	2	412243	7	NULL	NULL	0	NULL	long-term remissions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinico-dynamic aspects of long-term remissions in schizophrenia ) .
	manualset3
163916	3	412243	7	NULL	NULL	NULL	NULL	schizophrenia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Clinico-dynamic aspects of long-term remissions in schizophrenia ) .
	manualset3
163917	1	412244	7	NULL	NULL	0	NULL	Academic medicine amenities unit	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Academic medicine amenities unit : developing a model to integrate academic medical care with luxury hotel services .
	manualset3
163918	2	412244	7	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Academic medicine amenities unit : developing a model to integrate academic medical care with luxury hotel services .
	manualset3
163919	3	412244	7	NULL	NULL	0	NULL	academic medical care 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Academic medicine amenities unit : developing a model to integrate academic medical care with luxury hotel services .
	manualset3
163920	4	412244	7	NULL	NULL	0	NULL	 luxury hotel services	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Academic medicine amenities unit : developing a model to integrate academic medical care with luxury hotel services .
	manualset3
163921	1	412245	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of platelet transfusions depend upon a variety of different conditions ; besides alloimmunization , a lot of clinical factors are responsible for transfusion success .
	manualset3
163922	2	412245	7	NULL	NULL	0	NULL	platelet transfusions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of platelet transfusions depend upon a variety of different conditions ; besides alloimmunization , a lot of clinical factors are responsible for transfusion success .
	manualset3
163923	3	412245	7	NULL	NULL	0	NULL	conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of platelet transfusions depend upon a variety of different conditions ; besides alloimmunization , a lot of clinical factors are responsible for transfusion success .
	manualset3
163924	4	412245	7	NULL	NULL	0	NULL	alloimmunization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of platelet transfusions depend upon a variety of different conditions ; besides alloimmunization , a lot of clinical factors are responsible for transfusion success .
	manualset3
163925	5	412245	7	NULL	NULL	NULL	NULL	clinical factors	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of platelet transfusions depend upon a variety of different conditions ; besides alloimmunization , a lot of clinical factors are responsible for transfusion success .
	manualset3
163926	6	412245	7	NULL	NULL	0	NULL	transfusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of platelet transfusions depend upon a variety of different conditions ; besides alloimmunization , a lot of clinical factors are responsible for transfusion success .
	manualset3
163927	7	412245	7	NULL	NULL	0	NULL	success	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of platelet transfusions depend upon a variety of different conditions ; besides alloimmunization , a lot of clinical factors are responsible for transfusion success .
	manualset3
163928	1	412246	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of radiosensitizing activity of these agents against hypoxic Chinese hamster cells ( V-79 ) indicated that 2 , 4-dinitroimidazoles were better sensitizers than the nitroimidazo ( 2 , 1-b ) oxazoles , suggesting the necessity of the 2-nitro function in the molecule .
	manualset3
163929	2	412246	7	NULL	NULL	0	NULL	radiosensitizing activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of radiosensitizing activity of these agents against hypoxic Chinese hamster cells ( V-79 ) indicated that 2 , 4-dinitroimidazoles were better sensitizers than the nitroimidazo ( 2 , 1-b ) oxazoles , suggesting the necessity of the 2-nitro function in the molecule .
	manualset3
163930	3	412246	7	NULL	NULL	0	NULL	agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of radiosensitizing activity of these agents against hypoxic Chinese hamster cells ( V-79 ) indicated that 2 , 4-dinitroimidazoles were better sensitizers than the nitroimidazo ( 2 , 1-b ) oxazoles , suggesting the necessity of the 2-nitro function in the molecule .
	manualset3
163931	4	412246	7	NULL	NULL	0	NULL	 hypoxic Chinese hamster cells ( V-79 )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of radiosensitizing activity of these agents against hypoxic Chinese hamster cells ( V-79 ) indicated that 2 , 4-dinitroimidazoles were better sensitizers than the nitroimidazo ( 2 , 1-b ) oxazoles , suggesting the necessity of the 2-nitro function in the molecule .
	manualset3
163932	5	412246	7	NULL	NULL	0	NULL	2 , 4-dinitroimidazoles	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of radiosensitizing activity of these agents against hypoxic Chinese hamster cells ( V-79 ) indicated that 2 , 4-dinitroimidazoles were better sensitizers than the nitroimidazo ( 2 , 1-b ) oxazoles , suggesting the necessity of the 2-nitro function in the molecule .
	manualset3
163933	6	412246	7	NULL	NULL	0	NULL	sensitizers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of radiosensitizing activity of these agents against hypoxic Chinese hamster cells ( V-79 ) indicated that 2 , 4-dinitroimidazoles were better sensitizers than the nitroimidazo ( 2 , 1-b ) oxazoles , suggesting the necessity of the 2-nitro function in the molecule .
	manualset3
163934	7	412246	7	NULL	NULL	0	NULL	nitroimidazo ( 2 , 1-b ) oxazoles	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of radiosensitizing activity of these agents against hypoxic Chinese hamster cells ( V-79 ) indicated that 2 , 4-dinitroimidazoles were better sensitizers than the nitroimidazo ( 2 , 1-b ) oxazoles , suggesting the necessity of the 2-nitro function in the molecule .
	manualset3
163935	8	412246	7	NULL	NULL	0	NULL	 2-nitro function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of radiosensitizing activity of these agents against hypoxic Chinese hamster cells ( V-79 ) indicated that 2 , 4-dinitroimidazoles were better sensitizers than the nitroimidazo ( 2 , 1-b ) oxazoles , suggesting the necessity of the 2-nitro function in the molecule .
	manualset3
163936	9	412246	7	NULL	NULL	0	NULL	 molecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of radiosensitizing activity of these agents against hypoxic Chinese hamster cells ( V-79 ) indicated that 2 , 4-dinitroimidazoles were better sensitizers than the nitroimidazo ( 2 , 1-b ) oxazoles , suggesting the necessity of the 2-nitro function in the molecule .
	manualset3
163937	1	412247	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of reflex/motor activity interactions in 177 normal infants are evaluated .
	manualset3
163938	2	412247	7	NULL	NULL	0	NULL	reflex/motor activity interactions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of reflex/motor activity interactions in 177 normal infants are evaluated .
	manualset3
163939	3	412247	7	NULL	NULL	0	NULL	177 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of reflex/motor activity interactions in 177 normal infants are evaluated .
	manualset3
163940	4	412247	7	NULL	NULL	0	NULL	normal infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of reflex/motor activity interactions in 177 normal infants are evaluated .
	manualset3
163941	1	412248	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of the assays showed that the amounts of thromboxane and endothelin produced by endothelial cells in response to stimulation by hypertensive sera were significantly higher than the amounts produced in response to control sera ; in comparison , the amounts of prostacyclin and nitric oxide produced by the cells in response to either hypertensive sera or control sera were not significantly different .
	manualset3
163942	2	412248	7	NULL	NULL	0	NULL	assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the assays showed that the amounts of thromboxane and endothelin produced by endothelial cells in response to stimulation by hypertensive sera were significantly higher than the amounts produced in response to control sera ; in comparison , the amounts of prostacyclin and nitric oxide produced by the cells in response to either hypertensive sera or control sera were not significantly different .
	manualset3
163943	3	412248	7	NULL	NULL	0	NULL	amounts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the assays showed that the amounts of thromboxane and endothelin produced by endothelial cells in response to stimulation by hypertensive sera were significantly higher than the amounts produced in response to control sera ; in comparison , the amounts of prostacyclin and nitric oxide produced by the cells in response to either hypertensive sera or control sera were not significantly different .
	manualset3
163944	4	412248	7	NULL	NULL	0	NULL	thromboxane 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the assays showed that the amounts of thromboxane and endothelin produced by endothelial cells in response to stimulation by hypertensive sera were significantly higher than the amounts produced in response to control sera ; in comparison , the amounts of prostacyclin and nitric oxide produced by the cells in response to either hypertensive sera or control sera were not significantly different .
	manualset3
163945	5	412248	7	NULL	NULL	0	NULL	endothelin	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the assays showed that the amounts of thromboxane and endothelin produced by endothelial cells in response to stimulation by hypertensive sera were significantly higher than the amounts produced in response to control sera ; in comparison , the amounts of prostacyclin and nitric oxide produced by the cells in response to either hypertensive sera or control sera were not significantly different .
	manualset3
163946	6	412248	7	NULL	NULL	0	NULL	endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the assays showed that the amounts of thromboxane and endothelin produced by endothelial cells in response to stimulation by hypertensive sera were significantly higher than the amounts produced in response to control sera ; in comparison , the amounts of prostacyclin and nitric oxide produced by the cells in response to either hypertensive sera or control sera were not significantly different .
	manualset3
163947	7	412248	7	NULL	NULL	0	NULL	response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the assays showed that the amounts of thromboxane and endothelin produced by endothelial cells in response to stimulation by hypertensive sera were significantly higher than the amounts produced in response to control sera ; in comparison , the amounts of prostacyclin and nitric oxide produced by the cells in response to either hypertensive sera or control sera were not significantly different .
	manualset3
163948	8	412248	7	NULL	NULL	NULL	NULL	stimulation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of the assays showed that the amounts of thromboxane and endothelin produced by endothelial cells in response to stimulation by hypertensive sera were significantly higher than the amounts produced in response to control sera ; in comparison , the amounts of prostacyclin and nitric oxide produced by the cells in response to either hypertensive sera or control sera were not significantly different .
	manualset3
163949	9	412248	7	NULL	NULL	0	NULL	 hypertensive sera	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the assays showed that the amounts of thromboxane and endothelin produced by endothelial cells in response to stimulation by hypertensive sera were significantly higher than the amounts produced in response to control sera ; in comparison , the amounts of prostacyclin and nitric oxide produced by the cells in response to either hypertensive sera or control sera were not significantly different .
	manualset3
163950	10	412248	7	NULL	NULL	0	NULL	amounts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the assays showed that the amounts of thromboxane and endothelin produced by endothelial cells in response to stimulation by hypertensive sera were significantly higher than the amounts produced in response to control sera ; in comparison , the amounts of prostacyclin and nitric oxide produced by the cells in response to either hypertensive sera or control sera were not significantly different .
	manualset3
163951	11	412248	7	NULL	NULL	0	NULL	response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the assays showed that the amounts of thromboxane and endothelin produced by endothelial cells in response to stimulation by hypertensive sera were significantly higher than the amounts produced in response to control sera ; in comparison , the amounts of prostacyclin and nitric oxide produced by the cells in response to either hypertensive sera or control sera were not significantly different .
	manualset3
163952	12	412248	7	NULL	NULL	0	NULL	control sera	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the assays showed that the amounts of thromboxane and endothelin produced by endothelial cells in response to stimulation by hypertensive sera were significantly higher than the amounts produced in response to control sera ; in comparison , the amounts of prostacyclin and nitric oxide produced by the cells in response to either hypertensive sera or control sera were not significantly different .
	manualset3
163953	13	412248	7	NULL	NULL	0	NULL	 comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the assays showed that the amounts of thromboxane and endothelin produced by endothelial cells in response to stimulation by hypertensive sera were significantly higher than the amounts produced in response to control sera ; in comparison , the amounts of prostacyclin and nitric oxide produced by the cells in response to either hypertensive sera or control sera were not significantly different .
	manualset3
163954	14	412248	7	NULL	NULL	0	NULL	 amounts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the assays showed that the amounts of thromboxane and endothelin produced by endothelial cells in response to stimulation by hypertensive sera were significantly higher than the amounts produced in response to control sera ; in comparison , the amounts of prostacyclin and nitric oxide produced by the cells in response to either hypertensive sera or control sera were not significantly different .
	manualset3
163955	15	412248	7	NULL	NULL	0	NULL	prostacyclin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the assays showed that the amounts of thromboxane and endothelin produced by endothelial cells in response to stimulation by hypertensive sera were significantly higher than the amounts produced in response to control sera ; in comparison , the amounts of prostacyclin and nitric oxide produced by the cells in response to either hypertensive sera or control sera were not significantly different .
	manualset3
163956	16	412248	7	NULL	NULL	0	NULL	 nitric oxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the assays showed that the amounts of thromboxane and endothelin produced by endothelial cells in response to stimulation by hypertensive sera were significantly higher than the amounts produced in response to control sera ; in comparison , the amounts of prostacyclin and nitric oxide produced by the cells in response to either hypertensive sera or control sera were not significantly different .
	manualset3
163957	17	412248	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the assays showed that the amounts of thromboxane and endothelin produced by endothelial cells in response to stimulation by hypertensive sera were significantly higher than the amounts produced in response to control sera ; in comparison , the amounts of prostacyclin and nitric oxide produced by the cells in response to either hypertensive sera or control sera were not significantly different .
	manualset3
163958	18	412248	7	NULL	NULL	0	NULL	response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the assays showed that the amounts of thromboxane and endothelin produced by endothelial cells in response to stimulation by hypertensive sera were significantly higher than the amounts produced in response to control sera ; in comparison , the amounts of prostacyclin and nitric oxide produced by the cells in response to either hypertensive sera or control sera were not significantly different .
	manualset3
163959	19	412248	7	NULL	NULL	0	NULL	hypertensive sera	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the assays showed that the amounts of thromboxane and endothelin produced by endothelial cells in response to stimulation by hypertensive sera were significantly higher than the amounts produced in response to control sera ; in comparison , the amounts of prostacyclin and nitric oxide produced by the cells in response to either hypertensive sera or control sera were not significantly different .
	manualset3
163960	20	412248	7	NULL	NULL	0	NULL	control sera	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the assays showed that the amounts of thromboxane and endothelin produced by endothelial cells in response to stimulation by hypertensive sera were significantly higher than the amounts produced in response to control sera ; in comparison , the amounts of prostacyclin and nitric oxide produced by the cells in response to either hypertensive sera or control sera were not significantly different .
	manualset3
163961	1	412249	7	NULL	NULL	0	NULL	results	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the contralateral study show Nerisona cream and ointment to be more effective ( P less than 0.01 ) than Ultralan .
	manualset3
163962	2	412249	7	NULL	NULL	0	NULL	contralateral study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the contralateral study show Nerisona cream and ointment to be more effective ( P less than 0.01 ) than Ultralan .
	manualset3
163963	3	412249	7	NULL	NULL	0	NULL	Nerisona cream	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the contralateral study show Nerisona cream and ointment to be more effective ( P less than 0.01 ) than Ultralan .
	manualset3
163964	4	412249	7	NULL	NULL	0	NULL	ointment	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the contralateral study show Nerisona cream and ointment to be more effective ( P less than 0.01 ) than Ultralan .
	manualset3
163965	5	412249	7	NULL	NULL	0	NULL	P less than 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the contralateral study show Nerisona cream and ointment to be more effective ( P less than 0.01 ) than Ultralan .
	manualset3
163966	6	412249	7	NULL	NULL	0	NULL	Ultralan	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the contralateral study show Nerisona cream and ointment to be more effective ( P less than 0.01 ) than Ultralan .
	manualset3
163967	1	412250	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of the filter binding assay indicated that the primary binding target of HMG1 is the single-stranded region within the cruciform in supercoiled DNA .
	manualset3
163968	2	412250	7	NULL	NULL	0	NULL	 filter binding assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the filter binding assay indicated that the primary binding target of HMG1 is the single-stranded region within the cruciform in supercoiled DNA .
	manualset3
163969	3	412250	7	NULL	NULL	0	NULL	primary binding target	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the filter binding assay indicated that the primary binding target of HMG1 is the single-stranded region within the cruciform in supercoiled DNA .
	manualset3
163970	4	412250	7	NULL	NULL	0	NULL	HMG1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the filter binding assay indicated that the primary binding target of HMG1 is the single-stranded region within the cruciform in supercoiled DNA .
	manualset3
163971	5	412250	7	NULL	NULL	0	NULL	single-stranded region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the filter binding assay indicated that the primary binding target of HMG1 is the single-stranded region within the cruciform in supercoiled DNA .
	manualset3
163972	6	412250	7	NULL	NULL	0	NULL	 cruciform	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the filter binding assay indicated that the primary binding target of HMG1 is the single-stranded region within the cruciform in supercoiled DNA .
	manualset3
163973	7	412250	7	NULL	NULL	0	NULL	supercoiled DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the filter binding assay indicated that the primary binding target of HMG1 is the single-stranded region within the cruciform in supercoiled DNA .
	manualset3
163974	1	412251	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of the numerical simulations of ion beam extraction are found to be in good agreement with experimental data .
	manualset3
163975	2	412251	7	NULL	NULL	0	NULL	numerical simulations	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the numerical simulations of ion beam extraction are found to be in good agreement with experimental data .
	manualset3
163976	3	412251	7	NULL	NULL	0	NULL	ion beam extraction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the numerical simulations of ion beam extraction are found to be in good agreement with experimental data .
	manualset3
163977	4	412251	7	NULL	NULL	0	NULL	agreement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the numerical simulations of ion beam extraction are found to be in good agreement with experimental data .
	manualset3
163978	5	412251	7	NULL	NULL	0	NULL	experimental data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the numerical simulations of ion beam extraction are found to be in good agreement with experimental data .
	manualset3
163979	1	412252	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of the present study demonstrate that Polysorbate 80 is a proper vehicle for unravelling the reducing effect of Salvia miltiorrhiza extracts on alcohol intake .
	manualset3
163980	2	412252	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the present study demonstrate that Polysorbate 80 is a proper vehicle for unravelling the reducing effect of Salvia miltiorrhiza extracts on alcohol intake .
	manualset3
163981	3	412252	7	NULL	NULL	0	NULL	Polysorbate 80	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the present study demonstrate that Polysorbate 80 is a proper vehicle for unravelling the reducing effect of Salvia miltiorrhiza extracts on alcohol intake .
	manualset3
163982	4	412252	7	NULL	NULL	NULL	NULL	 vehicle	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of the present study demonstrate that Polysorbate 80 is a proper vehicle for unravelling the reducing effect of Salvia miltiorrhiza extracts on alcohol intake .
	manualset3
163983	5	412252	7	NULL	NULL	NULL	NULL	 unravelling	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of the present study demonstrate that Polysorbate 80 is a proper vehicle for unravelling the reducing effect of Salvia miltiorrhiza extracts on alcohol intake .
	manualset3
163984	6	412252	7	NULL	NULL	NULL	NULL	reducing effect 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of the present study demonstrate that Polysorbate 80 is a proper vehicle for unravelling the reducing effect of Salvia miltiorrhiza extracts on alcohol intake .
	manualset3
163985	7	412252	7	NULL	NULL	NULL	NULL	Salvia miltiorrhiza extracts	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of the present study demonstrate that Polysorbate 80 is a proper vehicle for unravelling the reducing effect of Salvia miltiorrhiza extracts on alcohol intake .
	manualset3
163986	8	412252	7	NULL	NULL	0	NULL	alcohol intake 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the present study demonstrate that Polysorbate 80 is a proper vehicle for unravelling the reducing effect of Salvia miltiorrhiza extracts on alcohol intake .
	manualset3
163987	1	412253	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of the present study emphasize that patients with ACS suffer from a definite rate of cardiac symptoms within the first month ( 63 % ) .
	manualset3
163988	2	412253	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the present study emphasize that patients with ACS suffer from a definite rate of cardiac symptoms within the first month ( 63 % ) .
	manualset3
163989	3	412253	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the present study emphasize that patients with ACS suffer from a definite rate of cardiac symptoms within the first month ( 63 % ) .
	manualset3
163990	4	412253	7	NULL	NULL	0	NULL	ACS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the present study emphasize that patients with ACS suffer from a definite rate of cardiac symptoms within the first month ( 63 % ) .
	manualset3
163991	5	412253	7	NULL	NULL	0	NULL	definite rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the present study emphasize that patients with ACS suffer from a definite rate of cardiac symptoms within the first month ( 63 % ) .
	manualset3
163992	6	412253	7	NULL	NULL	0	NULL	cardiac symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the present study emphasize that patients with ACS suffer from a definite rate of cardiac symptoms within the first month ( 63 % ) .
	manualset3
163993	7	412253	7	NULL	NULL	0	NULL	 first month	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the present study emphasize that patients with ACS suffer from a definite rate of cardiac symptoms within the first month ( 63 % ) .
	manualset3
163994	8	412253	7	NULL	NULL	0	NULL	63 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the present study emphasize that patients with ACS suffer from a definite rate of cardiac symptoms within the first month ( 63 % ) .
	manualset3
163995	1	412254	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of these analyses allowed us to map several known DNA fragments within deletion interval 6 in the following order : Ycen-pDP105B / 52dA , 50f2E , Fr25-II/Fr15-II , 50f2C , 49f-Yqter ( groups of fragments in undetermined order separated by diagonal lines ) .
	manualset3
163996	2	412254	7	NULL	NULL	0	NULL	analyses 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of these analyses allowed us to map several known DNA fragments within deletion interval 6 in the following order : Ycen-pDP105B / 52dA , 50f2E , Fr25-II/Fr15-II , 50f2C , 49f-Yqter ( groups of fragments in undetermined order separated by diagonal lines ) .
	manualset3
163997	3	412254	7	NULL	NULL	0	NULL	map 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of these analyses allowed us to map several known DNA fragments within deletion interval 6 in the following order : Ycen-pDP105B / 52dA , 50f2E , Fr25-II/Fr15-II , 50f2C , 49f-Yqter ( groups of fragments in undetermined order separated by diagonal lines ) .
	manualset3
163998	4	412254	7	NULL	NULL	0	NULL	DNA fragments	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of these analyses allowed us to map several known DNA fragments within deletion interval 6 in the following order : Ycen-pDP105B / 52dA , 50f2E , Fr25-II/Fr15-II , 50f2C , 49f-Yqter ( groups of fragments in undetermined order separated by diagonal lines ) .
	manualset3
163999	5	412254	7	NULL	NULL	0	NULL	deletion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of these analyses allowed us to map several known DNA fragments within deletion interval 6 in the following order : Ycen-pDP105B / 52dA , 50f2E , Fr25-II/Fr15-II , 50f2C , 49f-Yqter ( groups of fragments in undetermined order separated by diagonal lines ) .
	manualset3
164000	6	412254	7	NULL	NULL	NULL	NULL	interval 6	Chromosome												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of these analyses allowed us to map several known DNA fragments within deletion interval 6 in the following order : Ycen-pDP105B / 52dA , 50f2E , Fr25-II/Fr15-II , 50f2C , 49f-Yqter ( groups of fragments in undetermined order separated by diagonal lines ) .
	manualset3
164001	7	412254	7	NULL	NULL	0	NULL	order	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of these analyses allowed us to map several known DNA fragments within deletion interval 6 in the following order : Ycen-pDP105B / 52dA , 50f2E , Fr25-II/Fr15-II , 50f2C , 49f-Yqter ( groups of fragments in undetermined order separated by diagonal lines ) .
	manualset3
164002	8	412254	7	NULL	NULL	0	NULL	Ycen-pDP105B / 52dA	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of these analyses allowed us to map several known DNA fragments within deletion interval 6 in the following order : Ycen-pDP105B / 52dA , 50f2E , Fr25-II/Fr15-II , 50f2C , 49f-Yqter ( groups of fragments in undetermined order separated by diagonal lines ) .
	manualset3
164003	9	412254	7	NULL	NULL	0	NULL	50f2E	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of these analyses allowed us to map several known DNA fragments within deletion interval 6 in the following order : Ycen-pDP105B / 52dA , 50f2E , Fr25-II/Fr15-II , 50f2C , 49f-Yqter ( groups of fragments in undetermined order separated by diagonal lines ) .
	manualset3
164004	10	412254	7	NULL	NULL	0	NULL	Fr25-II/Fr15-II	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of these analyses allowed us to map several known DNA fragments within deletion interval 6 in the following order : Ycen-pDP105B / 52dA , 50f2E , Fr25-II/Fr15-II , 50f2C , 49f-Yqter ( groups of fragments in undetermined order separated by diagonal lines ) .
	manualset3
164005	11	412254	7	NULL	NULL	0	NULL	50f2C	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of these analyses allowed us to map several known DNA fragments within deletion interval 6 in the following order : Ycen-pDP105B / 52dA , 50f2E , Fr25-II/Fr15-II , 50f2C , 49f-Yqter ( groups of fragments in undetermined order separated by diagonal lines ) .
	manualset3
164006	12	412254	7	NULL	NULL	0	NULL	9f-Yqter	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of these analyses allowed us to map several known DNA fragments within deletion interval 6 in the following order : Ycen-pDP105B / 52dA , 50f2E , Fr25-II/Fr15-II , 50f2C , 49f-Yqter ( groups of fragments in undetermined order separated by diagonal lines ) .
	manualset3
164007	13	412254	7	NULL	NULL	0	NULL	groups of fragments	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of these analyses allowed us to map several known DNA fragments within deletion interval 6 in the following order : Ycen-pDP105B / 52dA , 50f2E , Fr25-II/Fr15-II , 50f2C , 49f-Yqter ( groups of fragments in undetermined order separated by diagonal lines ) .
	manualset3
164008	14	412254	7	NULL	NULL	0	NULL	order	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of these analyses allowed us to map several known DNA fragments within deletion interval 6 in the following order : Ycen-pDP105B / 52dA , 50f2E , Fr25-II/Fr15-II , 50f2C , 49f-Yqter ( groups of fragments in undetermined order separated by diagonal lines ) .
	manualset3
164009	15	412254	7	NULL	NULL	0	NULL	 diagonal lines	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of these analyses allowed us to map several known DNA fragments within deletion interval 6 in the following order : Ycen-pDP105B / 52dA , 50f2E , Fr25-II/Fr15-II , 50f2C , 49f-Yqter ( groups of fragments in undetermined order separated by diagonal lines ) .
	manualset3
164010	1	412255	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of these experiments indicate that simple gastrointestinal malaise in the absence of a deficiency state or acute toxemia will elicit pica .
	manualset3
164011	2	412255	7	NULL	NULL	0	NULL	experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of these experiments indicate that simple gastrointestinal malaise in the absence of a deficiency state or acute toxemia will elicit pica .
	manualset3
164012	3	412255	7	NULL	NULL	0	NULL	gastrointestinal malaise	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of these experiments indicate that simple gastrointestinal malaise in the absence of a deficiency state or acute toxemia will elicit pica .
	manualset3
164013	4	412255	7	NULL	NULL	0	NULL	 absence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of these experiments indicate that simple gastrointestinal malaise in the absence of a deficiency state or acute toxemia will elicit pica .
	manualset3
164014	5	412255	7	NULL	NULL	NULL	NULL	deficiency state	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of these experiments indicate that simple gastrointestinal malaise in the absence of a deficiency state or acute toxemia will elicit pica .
	manualset3
164015	6	412255	7	NULL	NULL	0	NULL	acute toxemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of these experiments indicate that simple gastrointestinal malaise in the absence of a deficiency state or acute toxemia will elicit pica .
	manualset3
164016	7	412255	7	NULL	NULL	0	NULL	pica	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of these experiments indicate that simple gastrointestinal malaise in the absence of a deficiency state or acute toxemia will elicit pica .
	manualset3
164017	1	412256	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of this study demonstrate a high prevalence of L. monocytogenes contamination in chicken carcasses , and all isolates were found to be sensitive to the antimicrobials most commonly used to treat human listeriosis .
	manualset3
164018	2	412256	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study demonstrate a high prevalence of L. monocytogenes contamination in chicken carcasses , and all isolates were found to be sensitive to the antimicrobials most commonly used to treat human listeriosis .
	manualset3
164019	3	412256	7	NULL	NULL	0	NULL	 high prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study demonstrate a high prevalence of L. monocytogenes contamination in chicken carcasses , and all isolates were found to be sensitive to the antimicrobials most commonly used to treat human listeriosis .
	manualset3
164020	4	412256	7	NULL	NULL	0	NULL	L. monocytogenes contamination	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study demonstrate a high prevalence of L. monocytogenes contamination in chicken carcasses , and all isolates were found to be sensitive to the antimicrobials most commonly used to treat human listeriosis .
	manualset3
164021	5	412256	7	NULL	NULL	0	NULL	chicken carcasses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study demonstrate a high prevalence of L. monocytogenes contamination in chicken carcasses , and all isolates were found to be sensitive to the antimicrobials most commonly used to treat human listeriosis .
	manualset3
164022	6	412256	7	NULL	NULL	NULL	NULL	isolates	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of this study demonstrate a high prevalence of L. monocytogenes contamination in chicken carcasses , and all isolates were found to be sensitive to the antimicrobials most commonly used to treat human listeriosis .
	manualset3
164023	7	412256	7	NULL	NULL	0	NULL	 antimicrobials 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study demonstrate a high prevalence of L. monocytogenes contamination in chicken carcasses , and all isolates were found to be sensitive to the antimicrobials most commonly used to treat human listeriosis .
	manualset3
164024	8	412256	7	NULL	NULL	NULL	NULL	human listeriosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of this study demonstrate a high prevalence of L. monocytogenes contamination in chicken carcasses , and all isolates were found to be sensitive to the antimicrobials most commonly used to treat human listeriosis .
	manualset3
164025	1	412257	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of this study document the rapid transition of this reef community from one in which corals and algae were codominant to a community dominated by macroalgae .
	manualset3
164026	2	412257	7	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study document the rapid transition of this reef community from one in which corals and algae were codominant to a community dominated by macroalgae .
	manualset3
164027	3	412257	7	NULL	NULL	NULL	NULL	rapid transition	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of this study document the rapid transition of this reef community from one in which corals and algae were codominant to a community dominated by macroalgae .
	manualset3
164028	4	412257	7	NULL	NULL	0	NULL	reef community	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study document the rapid transition of this reef community from one in which corals and algae were codominant to a community dominated by macroalgae .
	manualset3
164029	5	412257	7	NULL	NULL	0	NULL	 one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study document the rapid transition of this reef community from one in which corals and algae were codominant to a community dominated by macroalgae .
	manualset3
164030	6	412257	7	NULL	NULL	NULL	NULL	corals	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of this study document the rapid transition of this reef community from one in which corals and algae were codominant to a community dominated by macroalgae .
	manualset3
164031	7	412257	7	NULL	NULL	0	NULL	algae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study document the rapid transition of this reef community from one in which corals and algae were codominant to a community dominated by macroalgae .
	manualset3
164032	8	412257	7	NULL	NULL	0	NULL	community	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study document the rapid transition of this reef community from one in which corals and algae were codominant to a community dominated by macroalgae .
	manualset3
164033	9	412257	7	NULL	NULL	0	NULL	macroalgae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study document the rapid transition of this reef community from one in which corals and algae were codominant to a community dominated by macroalgae .
	manualset3
164034	1	412258	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of this study highlight some methodological and conceptual difficulties inherent to observational and geographical studies , in the specific context of the Portuguese population , and the challenge posed by the large numbers of pollutants considered .
	manualset3
164035	2	412258	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study highlight some methodological and conceptual difficulties inherent to observational and geographical studies , in the specific context of the Portuguese population , and the challenge posed by the large numbers of pollutants considered .
	manualset3
164036	3	412258	7	NULL	NULL	NULL	NULL	methodological difficulties	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of this study highlight some methodological and conceptual difficulties inherent to observational and geographical studies , in the specific context of the Portuguese population , and the challenge posed by the large numbers of pollutants considered .
	manualset3
164037	4	412258	7	NULL	NULL	NULL	NULL	conceptual difficulties	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of this study highlight some methodological and conceptual difficulties inherent to observational and geographical studies , in the specific context of the Portuguese population , and the challenge posed by the large numbers of pollutants considered .
	manualset3
164038	5	412258	7	NULL	NULL	0	NULL	observational studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study highlight some methodological and conceptual difficulties inherent to observational and geographical studies , in the specific context of the Portuguese population , and the challenge posed by the large numbers of pollutants considered .
	manualset3
164039	6	412258	7	NULL	NULL	0	NULL	geographical studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study highlight some methodological and conceptual difficulties inherent to observational and geographical studies , in the specific context of the Portuguese population , and the challenge posed by the large numbers of pollutants considered .
	manualset3
164040	7	412258	7	NULL	NULL	NULL	NULL	 context 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of this study highlight some methodological and conceptual difficulties inherent to observational and geographical studies , in the specific context of the Portuguese population , and the challenge posed by the large numbers of pollutants considered .
	manualset3
164041	8	412258	7	NULL	NULL	0	NULL	Portuguese population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study highlight some methodological and conceptual difficulties inherent to observational and geographical studies , in the specific context of the Portuguese population , and the challenge posed by the large numbers of pollutants considered .
	manualset3
164043	9	412258	7	NULL	NULL	NULL	NULL	challenge	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of this study highlight some methodological and conceptual difficulties inherent to observational and geographical studies , in the specific context of the Portuguese population , and the challenge posed by the large numbers of pollutants considered .
	manualset3
164044	10	412258	7	NULL	NULL	0	NULL	large numbers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study highlight some methodological and conceptual difficulties inherent to observational and geographical studies , in the specific context of the Portuguese population , and the challenge posed by the large numbers of pollutants considered .
	manualset3
164045	11	412258	7	NULL	NULL	0	NULL	 pollutants	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study highlight some methodological and conceptual difficulties inherent to observational and geographical studies , in the specific context of the Portuguese population , and the challenge posed by the large numbers of pollutants considered .
	manualset3
164046	1	412259	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of this study show increased SP and CGRP expression in the dorsal ganglia root cells of SHR compared to WKy rats .
	manualset3
164047	2	412259	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study show increased SP and CGRP expression in the dorsal ganglia root cells of SHR compared to WKy rats .
	manualset3
164048	3	412259	7	NULL	NULL	0	NULL	 increased SP expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study show increased SP and CGRP expression in the dorsal ganglia root cells of SHR compared to WKy rats .
	manualset3
164049	4	412259	7	NULL	NULL	0	NULL	increased CGRP expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study show increased SP and CGRP expression in the dorsal ganglia root cells of SHR compared to WKy rats .
	manualset3
164050	5	412259	7	NULL	NULL	0	NULL	dorsal ganglia root cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study show increased SP and CGRP expression in the dorsal ganglia root cells of SHR compared to WKy rats .
	manualset3
164051	6	412259	7	NULL	NULL	0	NULL	SHR	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study show increased SP and CGRP expression in the dorsal ganglia root cells of SHR compared to WKy rats .
	manualset3
164052	7	412259	7	NULL	NULL	0	NULL	WKy rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study show increased SP and CGRP expression in the dorsal ganglia root cells of SHR compared to WKy rats .
	manualset3
164053	1	412260	7	NULL	NULL	NULL	NULL	results 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of this study show that the presence of northern Entoloma species in Sicily is not influenced by the Mediterranean type of vegetation , by edaphic or altitudinal factors but by anomalous climatic trends of precipitations and temperatures which stimulate the fructification of basidiomata in correspondence with a thermal shock during autumn .
	manualset3
164054	2	412260	7	NULL	NULL	NULL	NULL	 study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of this study show that the presence of northern Entoloma species in Sicily is not influenced by the Mediterranean type of vegetation , by edaphic or altitudinal factors but by anomalous climatic trends of precipitations and temperatures which stimulate the fructification of basidiomata in correspondence with a thermal shock during autumn .
	manualset3
164055	3	412260	7	NULL	NULL	NULL	NULL	 presence	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of this study show that the presence of northern Entoloma species in Sicily is not influenced by the Mediterranean type of vegetation , by edaphic or altitudinal factors but by anomalous climatic trends of precipitations and temperatures which stimulate the fructification of basidiomata in correspondence with a thermal shock during autumn .
	manualset3
164056	4	412260	7	NULL	NULL	0	NULL	northern Entoloma species 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study show that the presence of northern Entoloma species in Sicily is not influenced by the Mediterranean type of vegetation , by edaphic or altitudinal factors but by anomalous climatic trends of precipitations and temperatures which stimulate the fructification of basidiomata in correspondence with a thermal shock during autumn .
	manualset3
164057	5	412260	7	NULL	NULL	0	NULL	Sicily	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study show that the presence of northern Entoloma species in Sicily is not influenced by the Mediterranean type of vegetation , by edaphic or altitudinal factors but by anomalous climatic trends of precipitations and temperatures which stimulate the fructification of basidiomata in correspondence with a thermal shock during autumn .
	manualset3
164058	6	412260	7	NULL	NULL	0	NULL	Mediterranean type	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study show that the presence of northern Entoloma species in Sicily is not influenced by the Mediterranean type of vegetation , by edaphic or altitudinal factors but by anomalous climatic trends of precipitations and temperatures which stimulate the fructification of basidiomata in correspondence with a thermal shock during autumn .
	manualset3
164059	7	412260	7	NULL	NULL	0	NULL	vegetation	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study show that the presence of northern Entoloma species in Sicily is not influenced by the Mediterranean type of vegetation , by edaphic or altitudinal factors but by anomalous climatic trends of precipitations and temperatures which stimulate the fructification of basidiomata in correspondence with a thermal shock during autumn .
	manualset3
164060	8	412260	7	NULL	NULL	0	NULL	edaphic factors	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study show that the presence of northern Entoloma species in Sicily is not influenced by the Mediterranean type of vegetation , by edaphic or altitudinal factors but by anomalous climatic trends of precipitations and temperatures which stimulate the fructification of basidiomata in correspondence with a thermal shock during autumn .
	manualset3
164061	9	412260	7	NULL	NULL	0	NULL	altitudinal factors	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study show that the presence of northern Entoloma species in Sicily is not influenced by the Mediterranean type of vegetation , by edaphic or altitudinal factors but by anomalous climatic trends of precipitations and temperatures which stimulate the fructification of basidiomata in correspondence with a thermal shock during autumn .
	manualset3
164062	10	412260	7	NULL	NULL	0	NULL	climatic trends	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study show that the presence of northern Entoloma species in Sicily is not influenced by the Mediterranean type of vegetation , by edaphic or altitudinal factors but by anomalous climatic trends of precipitations and temperatures which stimulate the fructification of basidiomata in correspondence with a thermal shock during autumn .
	manualset3
164063	11	412260	7	NULL	NULL	0	NULL	 precipitations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study show that the presence of northern Entoloma species in Sicily is not influenced by the Mediterranean type of vegetation , by edaphic or altitudinal factors but by anomalous climatic trends of precipitations and temperatures which stimulate the fructification of basidiomata in correspondence with a thermal shock during autumn .
	manualset3
164064	12	412260	7	NULL	NULL	0	NULL	temperatures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study show that the presence of northern Entoloma species in Sicily is not influenced by the Mediterranean type of vegetation , by edaphic or altitudinal factors but by anomalous climatic trends of precipitations and temperatures which stimulate the fructification of basidiomata in correspondence with a thermal shock during autumn .
	manualset3
164065	13	412260	7	NULL	NULL	0	NULL	fructification	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study show that the presence of northern Entoloma species in Sicily is not influenced by the Mediterranean type of vegetation , by edaphic or altitudinal factors but by anomalous climatic trends of precipitations and temperatures which stimulate the fructification of basidiomata in correspondence with a thermal shock during autumn .
	manualset3
164066	14	412260	7	NULL	NULL	0	NULL	basidiomata	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study show that the presence of northern Entoloma species in Sicily is not influenced by the Mediterranean type of vegetation , by edaphic or altitudinal factors but by anomalous climatic trends of precipitations and temperatures which stimulate the fructification of basidiomata in correspondence with a thermal shock during autumn .
	manualset3
164067	15	412260	7	NULL	NULL	0	NULL	 thermal shock	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study show that the presence of northern Entoloma species in Sicily is not influenced by the Mediterranean type of vegetation , by edaphic or altitudinal factors but by anomalous climatic trends of precipitations and temperatures which stimulate the fructification of basidiomata in correspondence with a thermal shock during autumn .
	manualset3
164068	16	412260	7	NULL	NULL	0	NULL	autumn	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study show that the presence of northern Entoloma species in Sicily is not influenced by the Mediterranean type of vegetation , by edaphic or altitudinal factors but by anomalous climatic trends of precipitations and temperatures which stimulate the fructification of basidiomata in correspondence with a thermal shock during autumn .
	manualset3
164069	1	412261	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggest that LVH in renovascular hypertension is associated with impairment in inotropic responsiveness to beta-receptor stimulation parallel with and , in part , related to , a reduction in ventricular beta-receptor concentrations .
	manualset3
164070	2	412261	7	NULL	NULL	NULL	NULL	 study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of this study suggest that LVH in renovascular hypertension is associated with impairment in inotropic responsiveness to beta-receptor stimulation parallel with and , in part , related to , a reduction in ventricular beta-receptor concentrations .
	manualset3
164071	3	412261	7	NULL	NULL	0	NULL	LVH	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggest that LVH in renovascular hypertension is associated with impairment in inotropic responsiveness to beta-receptor stimulation parallel with and , in part , related to , a reduction in ventricular beta-receptor concentrations .
	manualset3
164072	4	412261	7	NULL	NULL	0	NULL	renovascular hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggest that LVH in renovascular hypertension is associated with impairment in inotropic responsiveness to beta-receptor stimulation parallel with and , in part , related to , a reduction in ventricular beta-receptor concentrations .
	manualset3
164073	5	412261	7	NULL	NULL	0	NULL	impairment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggest that LVH in renovascular hypertension is associated with impairment in inotropic responsiveness to beta-receptor stimulation parallel with and , in part , related to , a reduction in ventricular beta-receptor concentrations .
	manualset3
164074	6	412261	7	NULL	NULL	0	NULL	inotropic responsiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggest that LVH in renovascular hypertension is associated with impairment in inotropic responsiveness to beta-receptor stimulation parallel with and , in part , related to , a reduction in ventricular beta-receptor concentrations .
	manualset3
164075	7	412261	7	NULL	NULL	0	NULL	beta-receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggest that LVH in renovascular hypertension is associated with impairment in inotropic responsiveness to beta-receptor stimulation parallel with and , in part , related to , a reduction in ventricular beta-receptor concentrations .
	manualset3
164076	8	412261	7	NULL	NULL	0	NULL	stimulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggest that LVH in renovascular hypertension is associated with impairment in inotropic responsiveness to beta-receptor stimulation parallel with and , in part , related to , a reduction in ventricular beta-receptor concentrations .
	manualset3
164077	9	412261	7	NULL	NULL	0	NULL	reduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggest that LVH in renovascular hypertension is associated with impairment in inotropic responsiveness to beta-receptor stimulation parallel with and , in part , related to , a reduction in ventricular beta-receptor concentrations .
	manualset3
164078	10	412261	7	NULL	NULL	0	NULL	ventricular beta-receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggest that LVH in renovascular hypertension is associated with impairment in inotropic responsiveness to beta-receptor stimulation parallel with and , in part , related to , a reduction in ventricular beta-receptor concentrations .
	manualset3
164079	11	412261	7	NULL	NULL	0	NULL	concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggest that LVH in renovascular hypertension is associated with impairment in inotropic responsiveness to beta-receptor stimulation parallel with and , in part , related to , a reduction in ventricular beta-receptor concentrations .
	manualset3
164080	1	412262	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of this study suggest that the observed increase in intracranial pressure during PHCA is not caused by increased cerebral perfusion , but rather that cerebral perfusion is reduced in response to a decreased demand for cerebral metabolic oxygen .
	manualset3
164081	2	412262	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggest that the observed increase in intracranial pressure during PHCA is not caused by increased cerebral perfusion , but rather that cerebral perfusion is reduced in response to a decreased demand for cerebral metabolic oxygen .
	manualset3
164082	3	412262	7	NULL	NULL	NULL	NULL	 increase	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of this study suggest that the observed increase in intracranial pressure during PHCA is not caused by increased cerebral perfusion , but rather that cerebral perfusion is reduced in response to a decreased demand for cerebral metabolic oxygen .
	manualset3
164083	4	412262	7	NULL	NULL	0	NULL	intracranial pressure 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggest that the observed increase in intracranial pressure during PHCA is not caused by increased cerebral perfusion , but rather that cerebral perfusion is reduced in response to a decreased demand for cerebral metabolic oxygen .
	manualset3
164084	5	412262	7	NULL	NULL	0	NULL	PHCA	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggest that the observed increase in intracranial pressure during PHCA is not caused by increased cerebral perfusion , but rather that cerebral perfusion is reduced in response to a decreased demand for cerebral metabolic oxygen .
	manualset3
164085	6	412262	7	NULL	NULL	0	NULL	increased cerebral perfusion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggest that the observed increase in intracranial pressure during PHCA is not caused by increased cerebral perfusion , but rather that cerebral perfusion is reduced in response to a decreased demand for cerebral metabolic oxygen .
	manualset3
164086	7	412262	7	NULL	NULL	0	NULL	cerebral perfusion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggest that the observed increase in intracranial pressure during PHCA is not caused by increased cerebral perfusion , but rather that cerebral perfusion is reduced in response to a decreased demand for cerebral metabolic oxygen .
	manualset3
164087	8	412262	7	NULL	NULL	0	NULL	response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggest that the observed increase in intracranial pressure during PHCA is not caused by increased cerebral perfusion , but rather that cerebral perfusion is reduced in response to a decreased demand for cerebral metabolic oxygen .
	manualset3
164088	9	412262	7	NULL	NULL	0	NULL	decreased demand	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggest that the observed increase in intracranial pressure during PHCA is not caused by increased cerebral perfusion , but rather that cerebral perfusion is reduced in response to a decreased demand for cerebral metabolic oxygen .
	manualset3
164089	10	412262	7	NULL	NULL	0	NULL	cerebral metabolic oxygen	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggest that the observed increase in intracranial pressure during PHCA is not caused by increased cerebral perfusion , but rather that cerebral perfusion is reduced in response to a decreased demand for cerebral metabolic oxygen .
	manualset3
164090	1	412263	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggested that body dissatisfaction and BDD among Turkish college students are not rare .
	manualset3
164091	2	412263	7	NULL	NULL	NULL	NULL	study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of this study suggested that body dissatisfaction and BDD among Turkish college students are not rare .
	manualset3
164092	3	412263	7	NULL	NULL	0	NULL	body dissatisfaction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggested that body dissatisfaction and BDD among Turkish college students are not rare .
	manualset3
164093	4	412263	7	NULL	NULL	0	NULL	BDD	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggested that body dissatisfaction and BDD among Turkish college students are not rare .
	manualset3
164094	5	412263	7	NULL	NULL	0	NULL	Turkish college students 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggested that body dissatisfaction and BDD among Turkish college students are not rare .
	manualset3
164095	1	412264	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of this study suggested that the kinin system may participate in the pathogenesis of human Ts envenomation and knowledge about this system may be useful to develop new strategies to reduce the damage caused by scorpion envenomation .
	manualset3
164096	2	412264	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggested that the kinin system may participate in the pathogenesis of human Ts envenomation and knowledge about this system may be useful to develop new strategies to reduce the damage caused by scorpion envenomation .
	manualset3
164097	3	412264	7	NULL	NULL	0	NULL	 kinin system 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggested that the kinin system may participate in the pathogenesis of human Ts envenomation and knowledge about this system may be useful to develop new strategies to reduce the damage caused by scorpion envenomation .
	manualset3
164098	4	412264	7	NULL	NULL	0	NULL	 pathogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggested that the kinin system may participate in the pathogenesis of human Ts envenomation and knowledge about this system may be useful to develop new strategies to reduce the damage caused by scorpion envenomation .
	manualset3
164099	5	412264	7	NULL	NULL	0	NULL	human Ts envenomation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggested that the kinin system may participate in the pathogenesis of human Ts envenomation and knowledge about this system may be useful to develop new strategies to reduce the damage caused by scorpion envenomation .
	manualset3
164100	6	412264	7	NULL	NULL	0	NULL	knowledge	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggested that the kinin system may participate in the pathogenesis of human Ts envenomation and knowledge about this system may be useful to develop new strategies to reduce the damage caused by scorpion envenomation .
	manualset3
164101	7	412264	7	NULL	NULL	0	NULL	system	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggested that the kinin system may participate in the pathogenesis of human Ts envenomation and knowledge about this system may be useful to develop new strategies to reduce the damage caused by scorpion envenomation .
	manualset3
164102	8	412264	7	NULL	NULL	0	NULL	new strategies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggested that the kinin system may participate in the pathogenesis of human Ts envenomation and knowledge about this system may be useful to develop new strategies to reduce the damage caused by scorpion envenomation .
	manualset3
164103	9	412264	7	NULL	NULL	0	NULL	damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggested that the kinin system may participate in the pathogenesis of human Ts envenomation and knowledge about this system may be useful to develop new strategies to reduce the damage caused by scorpion envenomation .
	manualset3
164104	10	412264	7	NULL	NULL	0	NULL	scorpion envenomation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this study suggested that the kinin system may participate in the pathogenesis of human Ts envenomation and knowledge about this system may be useful to develop new strategies to reduce the damage caused by scorpion envenomation .
	manualset3
164105	1	412265	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this treatment are positive , denoting the efficacy of PDT against chromoblastomycosis .
	manualset3
164106	2	412265	7	NULL	NULL	0	NULL	 treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this treatment are positive , denoting the efficacy of PDT against chromoblastomycosis .
	manualset3
164107	3	412265	7	NULL	NULL	0	NULL	efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this treatment are positive , denoting the efficacy of PDT against chromoblastomycosis .
	manualset3
164108	4	412265	7	NULL	NULL	0	NULL	PDT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this treatment are positive , denoting the efficacy of PDT against chromoblastomycosis .
	manualset3
164109	5	412265	7	NULL	NULL	0	NULL	chromoblastomycosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of this treatment are positive , denoting the efficacy of PDT against chromoblastomycosis .
	manualset3
164110	1	412266	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of treatment of 453 patients with grade 3 cervical intraepithelial neoplasia by cryotherapy are presented .
	manualset3
164111	2	412266	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of treatment of 453 patients with grade 3 cervical intraepithelial neoplasia by cryotherapy are presented .
	manualset3
164112	3	412266	7	NULL	NULL	0	NULL	453 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of treatment of 453 patients with grade 3 cervical intraepithelial neoplasia by cryotherapy are presented .
	manualset3
164113	4	412266	7	NULL	NULL	0	NULL	grade 3 cervical intraepithelial neoplasia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of treatment of 453 patients with grade 3 cervical intraepithelial neoplasia by cryotherapy are presented .
	manualset3
164114	5	412266	7	NULL	NULL	0	NULL	cryotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of treatment of 453 patients with grade 3 cervical intraepithelial neoplasia by cryotherapy are presented .
	manualset3
164115	1	412267	7	NULL	NULL	0	NULL	Acarbose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Acarbose acutely lowered post-prandial blood glucose and insulin area under the curve by a mean of 16.9 % and 9.2 % , respectively .
	manualset3
164116	2	412267	7	NULL	NULL	NULL	NULL	 post-prandial blood glucose	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Acarbose acutely lowered post-prandial blood glucose and insulin area under the curve by a mean of 16.9 % and 9.2 % , respectively .
	manualset3
164117	3	412267	7	NULL	NULL	NULL	NULL	insulin area	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Acarbose acutely lowered post-prandial blood glucose and insulin area under the curve by a mean of 16.9 % and 9.2 % , respectively .
	manualset3
164118	4	412267	7	NULL	NULL	0	NULL	curve 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Acarbose acutely lowered post-prandial blood glucose and insulin area under the curve by a mean of 16.9 % and 9.2 % , respectively .
	manualset3
164119	5	412267	7	NULL	NULL	0	NULL	mean	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Acarbose acutely lowered post-prandial blood glucose and insulin area under the curve by a mean of 16.9 % and 9.2 % , respectively .
	manualset3
164120	6	412267	7	NULL	NULL	0	NULL	16.9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Acarbose acutely lowered post-prandial blood glucose and insulin area under the curve by a mean of 16.9 % and 9.2 % , respectively .
	manualset3
164121	7	412267	7	NULL	NULL	0	NULL	9.2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Acarbose acutely lowered post-prandial blood glucose and insulin area under the curve by a mean of 16.9 % and 9.2 % , respectively .
	manualset3
164122	1	412268	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results pointed out that all dental bleaching agents tested contributed to DNA damage as depicted by the mean tail moment , being the strongest effect observed with the highest dose of hydrogen peroxide ( Whiteness HP and Lase Peroxide , at a 35 % concentration ) .
	manualset3
164123	2	412268	7	NULL	NULL	0	NULL	dental bleaching agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results pointed out that all dental bleaching agents tested contributed to DNA damage as depicted by the mean tail moment , being the strongest effect observed with the highest dose of hydrogen peroxide ( Whiteness HP and Lase Peroxide , at a 35 % concentration ) .
	manualset3
164124	3	412268	7	NULL	NULL	0	NULL	DNA damage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results pointed out that all dental bleaching agents tested contributed to DNA damage as depicted by the mean tail moment , being the strongest effect observed with the highest dose of hydrogen peroxide ( Whiteness HP and Lase Peroxide , at a 35 % concentration ) .
	manualset3
164125	4	412268	7	NULL	NULL	0	NULL	mean tail moment	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results pointed out that all dental bleaching agents tested contributed to DNA damage as depicted by the mean tail moment , being the strongest effect observed with the highest dose of hydrogen peroxide ( Whiteness HP and Lase Peroxide , at a 35 % concentration ) .
	manualset3
164126	5	412268	7	NULL	NULL	0	NULL	strongest effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results pointed out that all dental bleaching agents tested contributed to DNA damage as depicted by the mean tail moment , being the strongest effect observed with the highest dose of hydrogen peroxide ( Whiteness HP and Lase Peroxide , at a 35 % concentration ) .
	manualset3
164127	6	412268	7	NULL	NULL	0	NULL	highest dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results pointed out that all dental bleaching agents tested contributed to DNA damage as depicted by the mean tail moment , being the strongest effect observed with the highest dose of hydrogen peroxide ( Whiteness HP and Lase Peroxide , at a 35 % concentration ) .
	manualset3
164128	7	412268	7	NULL	NULL	0	NULL	hydrogen peroxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results pointed out that all dental bleaching agents tested contributed to DNA damage as depicted by the mean tail moment , being the strongest effect observed with the highest dose of hydrogen peroxide ( Whiteness HP and Lase Peroxide , at a 35 % concentration ) .
	manualset3
164129	8	412268	7	NULL	NULL	0	NULL	Whiteness HP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results pointed out that all dental bleaching agents tested contributed to DNA damage as depicted by the mean tail moment , being the strongest effect observed with the highest dose of hydrogen peroxide ( Whiteness HP and Lase Peroxide , at a 35 % concentration ) .
	manualset3
164130	9	412268	7	NULL	NULL	0	NULL	Lase Peroxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results pointed out that all dental bleaching agents tested contributed to DNA damage as depicted by the mean tail moment , being the strongest effect observed with the highest dose of hydrogen peroxide ( Whiteness HP and Lase Peroxide , at a 35 % concentration ) .
	manualset3
164131	10	412268	7	NULL	NULL	0	NULL	35 % concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results pointed out that all dental bleaching agents tested contributed to DNA damage as depicted by the mean tail moment , being the strongest effect observed with the highest dose of hydrogen peroxide ( Whiteness HP and Lase Peroxide , at a 35 % concentration ) .
	manualset3
164132	1	412269	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results presented here are used to further define the ACP ( Aerosol Collector Pyrolyser ) - GCMS experiment and provide a basis for modelling of aerosol composition on Titan and for the interpretation of Titan atmosphere data from the Huygens probe in the future .
	manualset3
164133	2	412269	7	NULL	NULL	0	NULL	ACP ( Aerosol Collector Pyrolyser ) - GCMS experiment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results presented here are used to further define the ACP ( Aerosol Collector Pyrolyser ) - GCMS experiment and provide a basis for modelling of aerosol composition on Titan and for the interpretation of Titan atmosphere data from the Huygens probe in the future .
	manualset3
164134	3	412269	7	NULL	NULL	0	NULL	basis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results presented here are used to further define the ACP ( Aerosol Collector Pyrolyser ) - GCMS experiment and provide a basis for modelling of aerosol composition on Titan and for the interpretation of Titan atmosphere data from the Huygens probe in the future .
	manualset3
164135	4	412269	7	NULL	NULL	0	NULL	modelling 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results presented here are used to further define the ACP ( Aerosol Collector Pyrolyser ) - GCMS experiment and provide a basis for modelling of aerosol composition on Titan and for the interpretation of Titan atmosphere data from the Huygens probe in the future .
	manualset3
164136	5	412269	7	NULL	NULL	0	NULL	aerosol composition	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results presented here are used to further define the ACP ( Aerosol Collector Pyrolyser ) - GCMS experiment and provide a basis for modelling of aerosol composition on Titan and for the interpretation of Titan atmosphere data from the Huygens probe in the future .
	manualset3
164137	6	412269	7	NULL	NULL	0	NULL	Titan	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results presented here are used to further define the ACP ( Aerosol Collector Pyrolyser ) - GCMS experiment and provide a basis for modelling of aerosol composition on Titan and for the interpretation of Titan atmosphere data from the Huygens probe in the future .
	manualset3
164138	7	412269	7	NULL	NULL	0	NULL	 interpretation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results presented here are used to further define the ACP ( Aerosol Collector Pyrolyser ) - GCMS experiment and provide a basis for modelling of aerosol composition on Titan and for the interpretation of Titan atmosphere data from the Huygens probe in the future .
	manualset3
164139	8	412269	7	NULL	NULL	0	NULL	Titan atmosphere data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The results presented here are used to further define the ACP ( Aerosol Collector Pyrolyser ) - GCMS experiment and provide a basis for modelling of aerosol composition on Titan and for the interpretation of Titan atmosphere data from the Huygens probe in the future .
	manualset3
164140	9	412269	7	NULL	NULL	NULL	NULL	Huygens probe	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results presented here are used to further define the ACP ( Aerosol Collector Pyrolyser ) - GCMS experiment and provide a basis for modelling of aerosol composition on Titan and for the interpretation of Titan atmosphere data from the Huygens probe in the future .
	manualset3
164141	1	412270	7	NULL	NULL	NULL	NULL	results 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results presented herein are consistent with a branched catalytic mechanism for the enzyme in which the ethylnitronate intermediate formed from the H196-catalyzed deprotonation of nitroethane partitions between release from the active site and oxidative denitrification to yield acetaldehyde and nitrite .
	manualset3
164142	2	412270	7	NULL	NULL	0	NULL	branched catalytic mechanism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results presented herein are consistent with a branched catalytic mechanism for the enzyme in which the ethylnitronate intermediate formed from the H196-catalyzed deprotonation of nitroethane partitions between release from the active site and oxidative denitrification to yield acetaldehyde and nitrite .
	manualset3
164143	3	412270	7	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results presented herein are consistent with a branched catalytic mechanism for the enzyme in which the ethylnitronate intermediate formed from the H196-catalyzed deprotonation of nitroethane partitions between release from the active site and oxidative denitrification to yield acetaldehyde and nitrite .
	manualset3
164144	4	412270	7	NULL	NULL	0	NULL	ethylnitronate intermediate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results presented herein are consistent with a branched catalytic mechanism for the enzyme in which the ethylnitronate intermediate formed from the H196-catalyzed deprotonation of nitroethane partitions between release from the active site and oxidative denitrification to yield acetaldehyde and nitrite .
	manualset3
164145	5	412270	7	NULL	NULL	0	NULL	H196-catalyzed deprotonation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results presented herein are consistent with a branched catalytic mechanism for the enzyme in which the ethylnitronate intermediate formed from the H196-catalyzed deprotonation of nitroethane partitions between release from the active site and oxidative denitrification to yield acetaldehyde and nitrite .
	manualset3
164146	6	412270	7	NULL	NULL	0	NULL	nitroethane partitions 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results presented herein are consistent with a branched catalytic mechanism for the enzyme in which the ethylnitronate intermediate formed from the H196-catalyzed deprotonation of nitroethane partitions between release from the active site and oxidative denitrification to yield acetaldehyde and nitrite .
	manualset3
164147	7	412270	7	NULL	NULL	0	NULL	release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results presented herein are consistent with a branched catalytic mechanism for the enzyme in which the ethylnitronate intermediate formed from the H196-catalyzed deprotonation of nitroethane partitions between release from the active site and oxidative denitrification to yield acetaldehyde and nitrite .
	manualset3
164148	8	412270	7	NULL	NULL	0	NULL	active site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results presented herein are consistent with a branched catalytic mechanism for the enzyme in which the ethylnitronate intermediate formed from the H196-catalyzed deprotonation of nitroethane partitions between release from the active site and oxidative denitrification to yield acetaldehyde and nitrite .
	manualset3
164149	9	412270	7	NULL	NULL	0	NULL	 oxidative denitrification	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results presented herein are consistent with a branched catalytic mechanism for the enzyme in which the ethylnitronate intermediate formed from the H196-catalyzed deprotonation of nitroethane partitions between release from the active site and oxidative denitrification to yield acetaldehyde and nitrite .
	manualset3
164150	10	412270	7	NULL	NULL	0	NULL	acetaldehyde	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results presented herein are consistent with a branched catalytic mechanism for the enzyme in which the ethylnitronate intermediate formed from the H196-catalyzed deprotonation of nitroethane partitions between release from the active site and oxidative denitrification to yield acetaldehyde and nitrite .
	manualset3
164151	11	412270	7	NULL	NULL	0	NULL	nitrite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results presented herein are consistent with a branched catalytic mechanism for the enzyme in which the ethylnitronate intermediate formed from the H196-catalyzed deprotonation of nitroethane partitions between release from the active site and oxidative denitrification to yield acetaldehyde and nitrite .
	manualset3
164157	1	412271	7	NULL	NULL	NULL	NULL	 results 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results presented in this paper indicate that NK-A receptors for neurokinins ( which are present in the tracheo-bronchial tree ) are also to be found in pulmonary vessels and mediate contraction of arterial vascular smooth muscle , an interesting property of neurokinins .
	manualset3
164158	2	412271	7	NULL	NULL	0	NULL	paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The results presented in this paper indicate that NK-A receptors for neurokinins ( which are present in the tracheo-bronchial tree ) are also to be found in pulmonary vessels and mediate contraction of arterial vascular smooth muscle , an interesting property of neurokinins .
	manualset3
164159	3	412271	7	NULL	NULL	0	NULL	NK-A receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results presented in this paper indicate that NK-A receptors for neurokinins ( which are present in the tracheo-bronchial tree ) are also to be found in pulmonary vessels and mediate contraction of arterial vascular smooth muscle , an interesting property of neurokinins .
	manualset3
164160	4	412271	7	NULL	NULL	0	NULL	neurokinins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results presented in this paper indicate that NK-A receptors for neurokinins ( which are present in the tracheo-bronchial tree ) are also to be found in pulmonary vessels and mediate contraction of arterial vascular smooth muscle , an interesting property of neurokinins .
	manualset3
164161	5	412271	7	NULL	NULL	0	NULL	tracheo-bronchial tree	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results presented in this paper indicate that NK-A receptors for neurokinins ( which are present in the tracheo-bronchial tree ) are also to be found in pulmonary vessels and mediate contraction of arterial vascular smooth muscle , an interesting property of neurokinins .
	manualset3
164162	6	412271	7	NULL	NULL	0	NULL	pulmonary vessels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results presented in this paper indicate that NK-A receptors for neurokinins ( which are present in the tracheo-bronchial tree ) are also to be found in pulmonary vessels and mediate contraction of arterial vascular smooth muscle , an interesting property of neurokinins .
	manualset3
164163	7	412271	7	NULL	NULL	0	NULL	contraction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results presented in this paper indicate that NK-A receptors for neurokinins ( which are present in the tracheo-bronchial tree ) are also to be found in pulmonary vessels and mediate contraction of arterial vascular smooth muscle , an interesting property of neurokinins .
	manualset3
164164	8	412271	7	NULL	NULL	NULL	NULL	arterial vascular smooth muscle	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results presented in this paper indicate that NK-A receptors for neurokinins ( which are present in the tracheo-bronchial tree ) are also to be found in pulmonary vessels and mediate contraction of arterial vascular smooth muscle , an interesting property of neurokinins .
	manualset3
164165	9	412271	7	NULL	NULL	0	NULL	interesting property	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results presented in this paper indicate that NK-A receptors for neurokinins ( which are present in the tracheo-bronchial tree ) are also to be found in pulmonary vessels and mediate contraction of arterial vascular smooth muscle , an interesting property of neurokinins .
	manualset3
164166	10	412271	7	NULL	NULL	0	NULL	neurokinins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results presented in this paper indicate that NK-A receptors for neurokinins ( which are present in the tracheo-bronchial tree ) are also to be found in pulmonary vessels and mediate contraction of arterial vascular smooth muscle , an interesting property of neurokinins .
	manualset3
164167	1	412272	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results provide important insight into the mechanism of papain digestion of mouse IgGs of different subclasses .
	manualset3
164168	2	412272	7	NULL	NULL	0	NULL	mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results provide important insight into the mechanism of papain digestion of mouse IgGs of different subclasses .
	manualset3
164169	3	412272	7	NULL	NULL	0	NULL	 papain digestion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results provide important insight into the mechanism of papain digestion of mouse IgGs of different subclasses .
	manualset3
164170	4	412272	7	NULL	NULL	0	NULL	mouse	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results provide important insight into the mechanism of papain digestion of mouse IgGs of different subclasses .
	manualset3
164171	5	412272	7	NULL	NULL	0	NULL	IgGs	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results provide important insight into the mechanism of papain digestion of mouse IgGs of different subclasses .
	manualset3
164172	6	412272	7	NULL	NULL	0	NULL	subclasses	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results provide important insight into the mechanism of papain digestion of mouse IgGs of different subclasses .
	manualset3
164173	1	412273	7	NULL	NULL	0	NULL	results 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results provide the first direct evidence in any species on the identification of specific cell surface receptors for a member of the GDF9/BMP15 subfamily of oocyte growth factors .
	manualset3
164174	2	412273	7	NULL	NULL	0	NULL	direct evidence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results provide the first direct evidence in any species on the identification of specific cell surface receptors for a member of the GDF9/BMP15 subfamily of oocyte growth factors .
	manualset3
164175	3	412273	7	NULL	NULL	0	NULL	species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results provide the first direct evidence in any species on the identification of specific cell surface receptors for a member of the GDF9/BMP15 subfamily of oocyte growth factors .
	manualset3
164176	4	412273	7	NULL	NULL	0	NULL	identification 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results provide the first direct evidence in any species on the identification of specific cell surface receptors for a member of the GDF9/BMP15 subfamily of oocyte growth factors .
	manualset3
164177	5	412273	7	NULL	NULL	0	NULL	cell surface receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results provide the first direct evidence in any species on the identification of specific cell surface receptors for a member of the GDF9/BMP15 subfamily of oocyte growth factors .
	manualset3
164178	6	412273	7	NULL	NULL	0	NULL	member	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results provide the first direct evidence in any species on the identification of specific cell surface receptors for a member of the GDF9/BMP15 subfamily of oocyte growth factors .
	manualset3
164179	7	412273	7	NULL	NULL	0	NULL	GDF9/BMP15 subfamily	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results provide the first direct evidence in any species on the identification of specific cell surface receptors for a member of the GDF9/BMP15 subfamily of oocyte growth factors .
	manualset3
164180	8	412273	7	NULL	NULL	0	NULL	oocyte growth factors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results provide the first direct evidence in any species on the identification of specific cell surface receptors for a member of the GDF9/BMP15 subfamily of oocyte growth factors .
	manualset3
164181	1	412274	7	NULL	NULL	0	NULL	Accelerated fractionation schedules	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Accelerated fractionation schedules were designed to counter accelerated repopulation .
	manualset3
164182	2	412274	7	NULL	NULL	NULL	NULL	accelerated repopulation	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Accelerated fractionation schedules were designed to counter accelerated repopulation .
	manualset3
164183	1	412275	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results show a distinct two stage perforation , thought to be the result of different mechanical properties of the layers in the arterial wall .
	manualset3
164184	2	412275	7	NULL	NULL	0	NULL	two stage perforation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show a distinct two stage perforation , thought to be the result of different mechanical properties of the layers in the arterial wall .
	manualset3
164185	3	412275	7	NULL	NULL	0	NULL	result 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show a distinct two stage perforation , thought to be the result of different mechanical properties of the layers in the arterial wall .
	manualset3
164186	4	412275	7	NULL	NULL	0	NULL	 mechanical properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show a distinct two stage perforation , thought to be the result of different mechanical properties of the layers in the arterial wall .
	manualset3
164187	5	412275	7	NULL	NULL	0	NULL	layers in the arterial wall	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show a distinct two stage perforation , thought to be the result of different mechanical properties of the layers in the arterial wall .
	manualset3
164188	1	412276	7	NULL	NULL	NULL	NULL	results 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results show that 76 % of the cows carrying the - LG AA genotype , 80 % of the cows carrying the - LG AB genotype , and 66 % of the cows carrying the - LG BB genotype were predicted correctly .
	manualset3
164189	2	412276	7	NULL	NULL	0	NULL	76 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that 76 % of the cows carrying the - LG AA genotype , 80 % of the cows carrying the - LG AB genotype , and 66 % of the cows carrying the - LG BB genotype were predicted correctly .
	manualset3
164190	3	412276	7	NULL	NULL	0	NULL	cows	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that 76 % of the cows carrying the - LG AA genotype , 80 % of the cows carrying the - LG AB genotype , and 66 % of the cows carrying the - LG BB genotype were predicted correctly .
	manualset3
164191	4	412276	7	NULL	NULL	NULL	NULL	 LG AA genotype	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results show that 76 % of the cows carrying the - LG AA genotype , 80 % of the cows carrying the - LG AB genotype , and 66 % of the cows carrying the - LG BB genotype were predicted correctly .
	manualset3
164192	5	412276	7	NULL	NULL	0	NULL	80 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that 76 % of the cows carrying the - LG AA genotype , 80 % of the cows carrying the - LG AB genotype , and 66 % of the cows carrying the - LG BB genotype were predicted correctly .
	manualset3
164193	6	412276	7	NULL	NULL	0	NULL	cows	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that 76 % of the cows carrying the - LG AA genotype , 80 % of the cows carrying the - LG AB genotype , and 66 % of the cows carrying the - LG BB genotype were predicted correctly .
	manualset3
164194	7	412276	7	NULL	NULL	NULL	NULL	LG AB genotype	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results show that 76 % of the cows carrying the - LG AA genotype , 80 % of the cows carrying the - LG AB genotype , and 66 % of the cows carrying the - LG BB genotype were predicted correctly .
	manualset3
164195	8	412276	7	NULL	NULL	0	NULL	66 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that 76 % of the cows carrying the - LG AA genotype , 80 % of the cows carrying the - LG AB genotype , and 66 % of the cows carrying the - LG BB genotype were predicted correctly .
	manualset3
164196	9	412276	7	NULL	NULL	0	NULL	 cows	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that 76 % of the cows carrying the - LG AA genotype , 80 % of the cows carrying the - LG AB genotype , and 66 % of the cows carrying the - LG BB genotype were predicted correctly .
	manualset3
164197	10	412276	7	NULL	NULL	NULL	NULL	LG BB genotype	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results show that 76 % of the cows carrying the - LG AA genotype , 80 % of the cows carrying the - LG AB genotype , and 66 % of the cows carrying the - LG BB genotype were predicted correctly .
	manualset3
164198	1	412277	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that LI is a useful tool for the treatment of tumor-bearing mice .
	manualset3
164199	2	412277	7	NULL	NULL	0	NULL	 LI 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that LI is a useful tool for the treatment of tumor-bearing mice .
	manualset3
164200	3	412277	7	NULL	NULL	0	NULL	tool 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that LI is a useful tool for the treatment of tumor-bearing mice .
	manualset3
164201	4	412277	7	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that LI is a useful tool for the treatment of tumor-bearing mice .
	manualset3
164202	5	412277	7	NULL	NULL	0	NULL	tumor-bearing mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that LI is a useful tool for the treatment of tumor-bearing mice .
	manualset3
164203	1	412278	7	NULL	NULL	0	NULL	 results 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that both BCK subunit protein and mRNA are upregulated early in myogenesis , and then downregulated in fully differentiated myotubes .
	manualset3
164204	2	412278	7	NULL	NULL	0	NULL	BCK subunit protein	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that both BCK subunit protein and mRNA are upregulated early in myogenesis , and then downregulated in fully differentiated myotubes .
	manualset3
164205	3	412278	7	NULL	NULL	0	NULL	mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that both BCK subunit protein and mRNA are upregulated early in myogenesis , and then downregulated in fully differentiated myotubes .
	manualset3
164206	4	412278	7	NULL	NULL	0	NULL	 early	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that both BCK subunit protein and mRNA are upregulated early in myogenesis , and then downregulated in fully differentiated myotubes .
	manualset3
164207	5	412278	7	NULL	NULL	0	NULL	myogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that both BCK subunit protein and mRNA are upregulated early in myogenesis , and then downregulated in fully differentiated myotubes .
	manualset3
164208	6	412278	7	NULL	NULL	0	NULL	 fully differentiated myotubes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that both BCK subunit protein and mRNA are upregulated early in myogenesis , and then downregulated in fully differentiated myotubes .
	manualset3
164209	1	412279	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that orexin A increases the sympathetic firing rate , IBAT and colonic temperatures and heart rate .
	manualset3
164210	2	412279	7	NULL	NULL	0	NULL	orexin A 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that orexin A increases the sympathetic firing rate , IBAT and colonic temperatures and heart rate .
	manualset3
164211	3	412279	7	NULL	NULL	NULL	NULL	sympathetic firing rate	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results show that orexin A increases the sympathetic firing rate , IBAT and colonic temperatures and heart rate .
	manualset3
164212	4	412279	7	NULL	NULL	NULL	NULL	 IBAT	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results show that orexin A increases the sympathetic firing rate , IBAT and colonic temperatures and heart rate .
	manualset3
164213	5	412279	7	NULL	NULL	NULL	NULL	colonic temperatures 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results show that orexin A increases the sympathetic firing rate , IBAT and colonic temperatures and heart rate .
	manualset3
164214	6	412279	7	NULL	NULL	NULL	NULL	heart rate	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results show that orexin A increases the sympathetic firing rate , IBAT and colonic temperatures and heart rate .
	manualset3
164215	1	412280	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results show that polyandry and in general flexibility in mating systems is a buffer mechanism that can significantly reduce the impact of environmental and demographic noise in small populations .
	manualset3
164216	2	412280	7	NULL	NULL	0	NULL	polyandry	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that polyandry and in general flexibility in mating systems is a buffer mechanism that can significantly reduce the impact of environmental and demographic noise in small populations .
	manualset3
164217	3	412280	7	NULL	NULL	NULL	NULL	 flexibility	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results show that polyandry and in general flexibility in mating systems is a buffer mechanism that can significantly reduce the impact of environmental and demographic noise in small populations .
	manualset3
164218	4	412280	7	NULL	NULL	0	NULL	mating systems	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that polyandry and in general flexibility in mating systems is a buffer mechanism that can significantly reduce the impact of environmental and demographic noise in small populations .
	manualset3
164219	5	412280	7	NULL	NULL	0	NULL	buffer mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that polyandry and in general flexibility in mating systems is a buffer mechanism that can significantly reduce the impact of environmental and demographic noise in small populations .
	manualset3
164220	6	412280	7	NULL	NULL	0	NULL	impact	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that polyandry and in general flexibility in mating systems is a buffer mechanism that can significantly reduce the impact of environmental and demographic noise in small populations .
	manualset3
164221	7	412280	7	NULL	NULL	0	NULL	environmental and demographic noise	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that polyandry and in general flexibility in mating systems is a buffer mechanism that can significantly reduce the impact of environmental and demographic noise in small populations .
	manualset3
164222	8	412280	7	NULL	NULL	0	NULL	small populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that polyandry and in general flexibility in mating systems is a buffer mechanism that can significantly reduce the impact of environmental and demographic noise in small populations .
	manualset3
165212	1	412281	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that protein of roasted wheat germs has higher digestibility ( D ) and protein efficiency ratio ( PER ) than the raw wheat germs which proves that roasting destroyed digestion enzymes inhibitors .
	manualset3
165213	2	412281	7	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that protein of roasted wheat germs has higher digestibility ( D ) and protein efficiency ratio ( PER ) than the raw wheat germs which proves that roasting destroyed digestion enzymes inhibitors .
	manualset3
165214	3	412281	7	NULL	NULL	0	NULL	 roasted wheat germs	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that protein of roasted wheat germs has higher digestibility ( D ) and protein efficiency ratio ( PER ) than the raw wheat germs which proves that roasting destroyed digestion enzymes inhibitors .
	manualset3
165215	4	412281	7	NULL	NULL	0	NULL	higher digestibility ( D )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that protein of roasted wheat germs has higher digestibility ( D ) and protein efficiency ratio ( PER ) than the raw wheat germs which proves that roasting destroyed digestion enzymes inhibitors .
	manualset3
165216	5	412281	7	NULL	NULL	0	NULL	 protein efficiency ratio ( PER )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that protein of roasted wheat germs has higher digestibility ( D ) and protein efficiency ratio ( PER ) than the raw wheat germs which proves that roasting destroyed digestion enzymes inhibitors .
	manualset3
165217	6	412281	7	NULL	NULL	0	NULL	raw wheat germs	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that protein of roasted wheat germs has higher digestibility ( D ) and protein efficiency ratio ( PER ) than the raw wheat germs which proves that roasting destroyed digestion enzymes inhibitors .
	manualset3
165218	7	412281	7	NULL	NULL	0	NULL	roasting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that protein of roasted wheat germs has higher digestibility ( D ) and protein efficiency ratio ( PER ) than the raw wheat germs which proves that roasting destroyed digestion enzymes inhibitors .
	manualset3
165219	8	412281	7	NULL	NULL	0	NULL	digestion enzyme inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that protein of roasted wheat germs has higher digestibility ( D ) and protein efficiency ratio ( PER ) than the raw wheat germs which proves that roasting destroyed digestion enzymes inhibitors .
	manualset3
164223	1	412282	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that the above described murine mAbs fragments do bind specifically to basophils obtained from allergic and nonallergic children .
	manualset3
164224	2	412282	7	NULL	NULL	0	NULL	murine mAbs fragments 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that the above described murine mAbs fragments do bind specifically to basophils obtained from allergic and nonallergic children .
	manualset3
164225	3	412282	7	NULL	NULL	0	NULL	basophils	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that the above described murine mAbs fragments do bind specifically to basophils obtained from allergic and nonallergic children .
	manualset3
164226	4	412282	7	NULL	NULL	0	NULL	allergic children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that the above described murine mAbs fragments do bind specifically to basophils obtained from allergic and nonallergic children .
	manualset3
164227	5	412282	7	NULL	NULL	0	NULL	nonallergic children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that the above described murine mAbs fragments do bind specifically to basophils obtained from allergic and nonallergic children .
	manualset3
164228	1	412283	7	NULL	NULL	0	NULL	Acceleration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acceleration of apoptosis in 3-oxo-C ( 12 ) - HSL-treated cells was confirmed by multiple criteria ( caspases 3 and 8 , histone-associated DNA fragments , phosphatidylserine expression ) .
	manualset3
164229	2	412283	7	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acceleration of apoptosis in 3-oxo-C ( 12 ) - HSL-treated cells was confirmed by multiple criteria ( caspases 3 and 8 , histone-associated DNA fragments , phosphatidylserine expression ) .
	manualset3
164230	3	412283	7	NULL	NULL	0	NULL	3-oxo-C ( 12 ) - HSL-treated cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Acceleration of apoptosis in 3-oxo-C ( 12 ) - HSL-treated cells was confirmed by multiple criteria ( caspases 3 and 8 , histone-associated DNA fragments , phosphatidylserine expression ) .
	manualset3
164231	4	412283	7	NULL	NULL	0	NULL	multiple criteria	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acceleration of apoptosis in 3-oxo-C ( 12 ) - HSL-treated cells was confirmed by multiple criteria ( caspases 3 and 8 , histone-associated DNA fragments , phosphatidylserine expression ) .
	manualset3
164232	5	412283	7	NULL	NULL	NULL	NULL	 caspases 3 expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Acceleration of apoptosis in 3-oxo-C ( 12 ) - HSL-treated cells was confirmed by multiple criteria ( caspases 3 and 8 , histone-associated DNA fragments , phosphatidylserine expression ) .
	manualset3
164233	6	412283	7	NULL	NULL	NULL	NULL	 caspases 8 expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Acceleration of apoptosis in 3-oxo-C ( 12 ) - HSL-treated cells was confirmed by multiple criteria ( caspases 3 and 8 , histone-associated DNA fragments , phosphatidylserine expression ) .
	manualset3
164234	7	412283	7	NULL	NULL	0	NULL	histone-associated DNA fragments	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Acceleration of apoptosis in 3-oxo-C ( 12 ) - HSL-treated cells was confirmed by multiple criteria ( caspases 3 and 8 , histone-associated DNA fragments , phosphatidylserine expression ) .
	manualset3
164235	8	412283	7	NULL	NULL	0	NULL	phosphatidylserine expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acceleration of apoptosis in 3-oxo-C ( 12 ) - HSL-treated cells was confirmed by multiple criteria ( caspases 3 and 8 , histone-associated DNA fragments , phosphatidylserine expression ) .
	manualset3
164236	1	412284	7	NULL	NULL	NULL	NULL	 results 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results show that the effects of adjusting from outdoor concentrations to personal exposures and correcting dose-response bias are nearly equal , so that roughly the same premature mortalities associated with short-term exposure to both ambient PM ( 2.5 ) and PM ( 10 ) in Los Angeles County are predicted with both models .
	manualset3
164237	2	412284	7	NULL	NULL	0	NULL	effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that the effects of adjusting from outdoor concentrations to personal exposures and correcting dose-response bias are nearly equal , so that roughly the same premature mortalities associated with short-term exposure to both ambient PM ( 2.5 ) and PM ( 10 ) in Los Angeles County are predicted with both models .
	manualset3
164238	3	412284	7	NULL	NULL	0	NULL	outdoor concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that the effects of adjusting from outdoor concentrations to personal exposures and correcting dose-response bias are nearly equal , so that roughly the same premature mortalities associated with short-term exposure to both ambient PM ( 2.5 ) and PM ( 10 ) in Los Angeles County are predicted with both models .
	manualset3
164239	4	412284	7	NULL	NULL	NULL	NULL	personal exposures	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results show that the effects of adjusting from outdoor concentrations to personal exposures and correcting dose-response bias are nearly equal , so that roughly the same premature mortalities associated with short-term exposure to both ambient PM ( 2.5 ) and PM ( 10 ) in Los Angeles County are predicted with both models .
	manualset3
164240	5	412284	7	NULL	NULL	0	NULL	dose-response bias	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that the effects of adjusting from outdoor concentrations to personal exposures and correcting dose-response bias are nearly equal , so that roughly the same premature mortalities associated with short-term exposure to both ambient PM ( 2.5 ) and PM ( 10 ) in Los Angeles County are predicted with both models .
	manualset3
164241	6	412284	7	NULL	NULL	0	NULL	premature mortalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that the effects of adjusting from outdoor concentrations to personal exposures and correcting dose-response bias are nearly equal , so that roughly the same premature mortalities associated with short-term exposure to both ambient PM ( 2.5 ) and PM ( 10 ) in Los Angeles County are predicted with both models .
	manualset3
164242	7	412284	7	NULL	NULL	0	NULL	short-term exposure 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that the effects of adjusting from outdoor concentrations to personal exposures and correcting dose-response bias are nearly equal , so that roughly the same premature mortalities associated with short-term exposure to both ambient PM ( 2.5 ) and PM ( 10 ) in Los Angeles County are predicted with both models .
	manualset3
164243	8	412284	7	NULL	NULL	0	NULL	ambient PM ( 2.5 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that the effects of adjusting from outdoor concentrations to personal exposures and correcting dose-response bias are nearly equal , so that roughly the same premature mortalities associated with short-term exposure to both ambient PM ( 2.5 ) and PM ( 10 ) in Los Angeles County are predicted with both models .
	manualset3
164244	9	412284	7	NULL	NULL	0	NULL	PM ( 10 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that the effects of adjusting from outdoor concentrations to personal exposures and correcting dose-response bias are nearly equal , so that roughly the same premature mortalities associated with short-term exposure to both ambient PM ( 2.5 ) and PM ( 10 ) in Los Angeles County are predicted with both models .
	manualset3
164245	10	412284	7	NULL	NULL	0	NULL	Los Angeles County	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that the effects of adjusting from outdoor concentrations to personal exposures and correcting dose-response bias are nearly equal , so that roughly the same premature mortalities associated with short-term exposure to both ambient PM ( 2.5 ) and PM ( 10 ) in Los Angeles County are predicted with both models .
	manualset3
164246	11	412284	7	NULL	NULL	0	NULL	models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that the effects of adjusting from outdoor concentrations to personal exposures and correcting dose-response bias are nearly equal , so that roughly the same premature mortalities associated with short-term exposure to both ambient PM ( 2.5 ) and PM ( 10 ) in Los Angeles County are predicted with both models .
	manualset3
164247	1	412285	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results show that the fusion protein exists in the physiological form as a dimer , has the ability to bind with TNF and inhibits the cytotoxicity of TNF on L929 cells .
	manualset3
164248	2	412285	7	NULL	NULL	0	NULL	fusion protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that the fusion protein exists in the physiological form as a dimer , has the ability to bind with TNF and inhibits the cytotoxicity of TNF on L929 cells .
	manualset3
164249	3	412285	7	NULL	NULL	0	NULL	 physiological form	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that the fusion protein exists in the physiological form as a dimer , has the ability to bind with TNF and inhibits the cytotoxicity of TNF on L929 cells .
	manualset3
164250	4	412285	7	NULL	NULL	0	NULL	 dimer	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that the fusion protein exists in the physiological form as a dimer , has the ability to bind with TNF and inhibits the cytotoxicity of TNF on L929 cells .
	manualset3
164251	5	412285	7	NULL	NULL	0	NULL	ability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that the fusion protein exists in the physiological form as a dimer , has the ability to bind with TNF and inhibits the cytotoxicity of TNF on L929 cells .
	manualset3
164252	6	412285	7	NULL	NULL	0	NULL	 TNF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that the fusion protein exists in the physiological form as a dimer , has the ability to bind with TNF and inhibits the cytotoxicity of TNF on L929 cells .
	manualset3
164253	7	412285	7	NULL	NULL	0	NULL	cytotoxicity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that the fusion protein exists in the physiological form as a dimer , has the ability to bind with TNF and inhibits the cytotoxicity of TNF on L929 cells .
	manualset3
164254	8	412285	7	NULL	NULL	0	NULL	TNF 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that the fusion protein exists in the physiological form as a dimer , has the ability to bind with TNF and inhibits the cytotoxicity of TNF on L929 cells .
	manualset3
164255	9	412285	7	NULL	NULL	0	NULL	L929 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that the fusion protein exists in the physiological form as a dimer , has the ability to bind with TNF and inhibits the cytotoxicity of TNF on L929 cells .
	manualset3
164256	1	412286	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results show that the most critical threat for the THIS is power failure followed by acts of human error or failure and other technological factors .
	manualset3
164257	2	412286	7	NULL	NULL	0	NULL	critical threat	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that the most critical threat for the THIS is power failure followed by acts of human error or failure and other technological factors .
	manualset3
164258	3	412286	7	NULL	NULL	0	NULL	THIS	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that the most critical threat for the THIS is power failure followed by acts of human error or failure and other technological factors .
	manualset3
164259	4	412286	7	NULL	NULL	0	NULL	power failure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that the most critical threat for the THIS is power failure followed by acts of human error or failure and other technological factors .
	manualset3
164260	5	412286	7	NULL	NULL	NULL	NULL	human error or failure	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results show that the most critical threat for the THIS is power failure followed by acts of human error or failure and other technological factors .
	manualset3
164261	6	412286	7	NULL	NULL	0	NULL	technological factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that the most critical threat for the THIS is power failure followed by acts of human error or failure and other technological factors .
	manualset3
164262	1	412287	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that walls of coronary arteries as small as 45 m in diameter are visible using a table-top micro-CT scanner .
	manualset3
164263	2	412287	7	NULL	NULL	0	NULL	walls of coronary arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that walls of coronary arteries as small as 45 m in diameter are visible using a table-top micro-CT scanner .
	manualset3
164264	3	412287	7	NULL	NULL	0	NULL	45 m	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that walls of coronary arteries as small as 45 m in diameter are visible using a table-top micro-CT scanner .
	manualset3
164265	4	412287	7	NULL	NULL	NULL	NULL	diameter	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results show that walls of coronary arteries as small as 45 m in diameter are visible using a table-top micro-CT scanner .
	manualset3
164266	5	412287	7	NULL	NULL	0	NULL	table-top micro-CT scanner	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that walls of coronary arteries as small as 45 m in diameter are visible using a table-top micro-CT scanner .
	manualset3
164268	1	412288	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that when the motor neuron is active at 20 impulses/second , it releases 50 quanta/impulse per muscle fiber , or a total of 4.5 x 10 ( 9 ) quanta/hr .
	manualset3
164269	2	412288	7	NULL	NULL	0	NULL	motor neuron	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that when the motor neuron is active at 20 impulses/second , it releases 50 quanta/impulse per muscle fiber , or a total of 4.5 x 10 ( 9 ) quanta/hr .
	manualset3
164270	3	412288	7	NULL	NULL	0	NULL	20 impulses/second	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that when the motor neuron is active at 20 impulses/second , it releases 50 quanta/impulse per muscle fiber , or a total of 4.5 x 10 ( 9 ) quanta/hr .
	manualset3
164271	4	412288	7	NULL	NULL	0	NULL	50 quanta/impulse per muscle fiber	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that when the motor neuron is active at 20 impulses/second , it releases 50 quanta/impulse per muscle fiber , or a total of 4.5 x 10 ( 9 ) quanta/hr .
	manualset3
164272	5	412288	7	NULL	NULL	0	NULL	4.5 x 10 ( 9 ) quanta/hr	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that when the motor neuron is active at 20 impulses/second , it releases 50 quanta/impulse per muscle fiber , or a total of 4.5 x 10 ( 9 ) quanta/hr .
	manualset3
164273	1	412289	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed a significant activation of apoptotic pathway as analyzed by caspase-3 induction as well as the expression of CHOP , a downstream effector of GCN2 kinase pathway in T cells , but not in skin cells .
	manualset3
164274	2	412289	7	NULL	NULL	NULL	NULL	activation 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed a significant activation of apoptotic pathway as analyzed by caspase-3 induction as well as the expression of CHOP , a downstream effector of GCN2 kinase pathway in T cells , but not in skin cells .
	manualset3
164275	3	412289	7	NULL	NULL	NULL	NULL	apoptotic pathway	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed a significant activation of apoptotic pathway as analyzed by caspase-3 induction as well as the expression of CHOP , a downstream effector of GCN2 kinase pathway in T cells , but not in skin cells .
	manualset3
164276	4	412289	7	NULL	NULL	0	NULL	caspase-3 induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed a significant activation of apoptotic pathway as analyzed by caspase-3 induction as well as the expression of CHOP , a downstream effector of GCN2 kinase pathway in T cells , but not in skin cells .
	manualset3
164277	5	412289	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed a significant activation of apoptotic pathway as analyzed by caspase-3 induction as well as the expression of CHOP , a downstream effector of GCN2 kinase pathway in T cells , but not in skin cells .
	manualset3
164278	6	412289	7	NULL	NULL	0	NULL	CHOP 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed a significant activation of apoptotic pathway as analyzed by caspase-3 induction as well as the expression of CHOP , a downstream effector of GCN2 kinase pathway in T cells , but not in skin cells .
	manualset3
164279	7	412289	7	NULL	NULL	0	NULL	downstream effector 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed a significant activation of apoptotic pathway as analyzed by caspase-3 induction as well as the expression of CHOP , a downstream effector of GCN2 kinase pathway in T cells , but not in skin cells .
	manualset3
164280	8	412289	7	NULL	NULL	0	NULL	GCN2 kinase pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed a significant activation of apoptotic pathway as analyzed by caspase-3 induction as well as the expression of CHOP , a downstream effector of GCN2 kinase pathway in T cells , but not in skin cells .
	manualset3
164281	9	412289	7	NULL	NULL	0	NULL	T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed a significant activation of apoptotic pathway as analyzed by caspase-3 induction as well as the expression of CHOP , a downstream effector of GCN2 kinase pathway in T cells , but not in skin cells .
	manualset3
164282	10	412289	7	NULL	NULL	0	NULL	skin cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed a significant activation of apoptotic pathway as analyzed by caspase-3 induction as well as the expression of CHOP , a downstream effector of GCN2 kinase pathway in T cells , but not in skin cells .
	manualset3
164283	1	412290	7	NULL	NULL	NULL	NULL	 results 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed a statistically significant post-dialysis increase in lipase only when heparin was used ( p & lt ; 0.03 ) .
	manualset3
164284	2	412290	7	NULL	NULL	0	NULL	post-dialysis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed a statistically significant post-dialysis increase in lipase only when heparin was used ( p & lt ; 0.03 ) .
	manualset3
164285	3	412290	7	NULL	NULL	NULL	NULL	 increase	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed a statistically significant post-dialysis increase in lipase only when heparin was used ( p & lt ; 0.03 ) .
	manualset3
164286	4	412290	7	NULL	NULL	0	NULL	lipase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed a statistically significant post-dialysis increase in lipase only when heparin was used ( p & lt ; 0.03 ) .
	manualset3
164287	5	412290	7	NULL	NULL	0	NULL	heparin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed a statistically significant post-dialysis increase in lipase only when heparin was used ( p & lt ; 0.03 ) .
	manualset3
164288	6	412290	7	NULL	NULL	0	NULL	p & lt ; 0.03	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed a statistically significant post-dialysis increase in lipase only when heparin was used ( p & lt ; 0.03 ) .
	manualset3
164289	1	412291	7	NULL	NULL	0	NULL	Acceleration 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acceleration of the CDP-ethanolamine pathway also does not change the rate of PtdEtn formation via the decarboxylation of phosphatidylserine .
	manualset3
164290	2	412291	7	NULL	NULL	0	NULL	CDP-ethanolamine pathway 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acceleration of the CDP-ethanolamine pathway also does not change the rate of PtdEtn formation via the decarboxylation of phosphatidylserine .
	manualset3
164291	3	412291	7	NULL	NULL	0	NULL	rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Acceleration of the CDP-ethanolamine pathway also does not change the rate of PtdEtn formation via the decarboxylation of phosphatidylserine .
	manualset3
164292	4	412291	7	NULL	NULL	0	NULL	PtdEtn formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acceleration of the CDP-ethanolamine pathway also does not change the rate of PtdEtn formation via the decarboxylation of phosphatidylserine .
	manualset3
164293	5	412291	7	NULL	NULL	0	NULL	decarboxylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acceleration of the CDP-ethanolamine pathway also does not change the rate of PtdEtn formation via the decarboxylation of phosphatidylserine .
	manualset3
164294	6	412291	7	NULL	NULL	0	NULL	phosphatidylserine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Acceleration of the CDP-ethanolamine pathway also does not change the rate of PtdEtn formation via the decarboxylation of phosphatidylserine .
	manualset3
164295	1	412292	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed an increase of moisture and protein contents after the fat replacement , while the fat reduction of 25-35 % led to the preparation of light products .
	manualset3
164296	2	412292	7	NULL	NULL	NULL	NULL	increase	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed an increase of moisture and protein contents after the fat replacement , while the fat reduction of 25-35 % led to the preparation of light products .
	manualset3
164297	3	412292	7	NULL	NULL	0	NULL	moisture contents	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed an increase of moisture and protein contents after the fat replacement , while the fat reduction of 25-35 % led to the preparation of light products .
	manualset3
164298	4	412292	7	NULL	NULL	0	NULL	protein contents	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed an increase of moisture and protein contents after the fat replacement , while the fat reduction of 25-35 % led to the preparation of light products .
	manualset3
164299	5	412292	7	NULL	NULL	NULL	NULL	fat replacement	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed an increase of moisture and protein contents after the fat replacement , while the fat reduction of 25-35 % led to the preparation of light products .
	manualset3
164300	6	412292	7	NULL	NULL	0	NULL	 fat reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed an increase of moisture and protein contents after the fat replacement , while the fat reduction of 25-35 % led to the preparation of light products .
	manualset3
164301	7	412292	7	NULL	NULL	0	NULL	25-35 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed an increase of moisture and protein contents after the fat replacement , while the fat reduction of 25-35 % led to the preparation of light products .
	manualset3
164302	8	412292	7	NULL	NULL	0	NULL	preparation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed an increase of moisture and protein contents after the fat replacement , while the fat reduction of 25-35 % led to the preparation of light products .
	manualset3
164303	9	412292	7	NULL	NULL	0	NULL	light products	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed an increase of moisture and protein contents after the fat replacement , while the fat reduction of 25-35 % led to the preparation of light products .
	manualset3
164304	1	412293	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed significant ( P less than 0.0001 ) protection afforded by BBI against peroxidation at 1.16 ( 65 % ) , 1.93 ( 60 % , and 2.70 ( 48 % ) J/m2 of UVC irradiation .
	manualset3
164305	2	412293	7	NULL	NULL	0	NULL	P less than 0.0001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed significant ( P less than 0.0001 ) protection afforded by BBI against peroxidation at 1.16 ( 65 % ) , 1.93 ( 60 % , and 2.70 ( 48 % ) J/m2 of UVC irradiation .
	manualset3
164306	3	412293	7	NULL	NULL	0	NULL	protection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed significant ( P less than 0.0001 ) protection afforded by BBI against peroxidation at 1.16 ( 65 % ) , 1.93 ( 60 % , and 2.70 ( 48 % ) J/m2 of UVC irradiation .
	manualset3
164307	4	412293	7	NULL	NULL	0	NULL	BBI	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed significant ( P less than 0.0001 ) protection afforded by BBI against peroxidation at 1.16 ( 65 % ) , 1.93 ( 60 % , and 2.70 ( 48 % ) J/m2 of UVC irradiation .
	manualset3
164308	5	412293	7	NULL	NULL	0	NULL	 peroxidation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed significant ( P less than 0.0001 ) protection afforded by BBI against peroxidation at 1.16 ( 65 % ) , 1.93 ( 60 % , and 2.70 ( 48 % ) J/m2 of UVC irradiation .
	manualset3
164309	6	412293	7	NULL	NULL	0	NULL	1.16 ( 65 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed significant ( P less than 0.0001 ) protection afforded by BBI against peroxidation at 1.16 ( 65 % ) , 1.93 ( 60 % , and 2.70 ( 48 % ) J/m2 of UVC irradiation .
	manualset3
164310	7	412293	7	NULL	NULL	NULL	NULL	1.93 ( 60 % )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed significant ( P less than 0.0001 ) protection afforded by BBI against peroxidation at 1.16 ( 65 % ) , 1.93 ( 60 % , and 2.70 ( 48 % ) J/m2 of UVC irradiation .
	manualset3
164311	9	412293	7	NULL	NULL	NULL	NULL	J/m2	Unit												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed significant ( P less than 0.0001 ) protection afforded by BBI against peroxidation at 1.16 ( 65 % ) , 1.93 ( 60 % , and 2.70 ( 48 % ) J/m2 of UVC irradiation .
	manualset3
164312	10	412293	7	NULL	NULL	NULL	NULL	UVC irradiation	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed significant ( P less than 0.0001 ) protection afforded by BBI against peroxidation at 1.16 ( 65 % ) , 1.93 ( 60 % , and 2.70 ( 48 % ) J/m2 of UVC irradiation .
	manualset3
164313	8	412293	7	NULL	NULL	0	NULL	2.70 ( 48 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed significant ( P less than 0.0001 ) protection afforded by BBI against peroxidation at 1.16 ( 65 % ) , 1.93 ( 60 % , and 2.70 ( 48 % ) J/m2 of UVC irradiation .
	manualset3
164314	1	412294	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed that 1 out of 7 chicken samples contained over 30 ng/g of NCZ .
	manualset3
164315	2	412294	7	NULL	NULL	0	NULL	1 out of 7	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that 1 out of 7 chicken samples contained over 30 ng/g of NCZ .
	manualset3
164316	3	412294	7	NULL	NULL	0	NULL	chicken samples	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that 1 out of 7 chicken samples contained over 30 ng/g of NCZ .
	manualset3
164317	4	412294	7	NULL	NULL	0	NULL	30 ng/g	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that 1 out of 7 chicken samples contained over 30 ng/g of NCZ .
	manualset3
164318	5	412294	7	NULL	NULL	0	NULL	NCZ	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that 1 out of 7 chicken samples contained over 30 ng/g of NCZ .
	manualset3
164319	1	412295	7	NULL	NULL	NULL	NULL	results 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed that 18 preparations contained antibiotic substances in an amount of 0.6-1300 U , equivalent to oxytetracycline units per 1 g. Most often antibiotics were present in preparations of the pectinase and protease group .
	manualset3
164320	2	412295	7	NULL	NULL	NULL	NULL	18 preparations	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed that 18 preparations contained antibiotic substances in an amount of 0.6-1300 U , equivalent to oxytetracycline units per 1 g. Most often antibiotics were present in preparations of the pectinase and protease group .
	manualset3
164321	3	412295	7	NULL	NULL	0	NULL	 antibiotic substances	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that 18 preparations contained antibiotic substances in an amount of 0.6-1300 U , equivalent to oxytetracycline units per 1 g. Most often antibiotics were present in preparations of the pectinase and protease group .
	manualset3
164322	4	412295	7	NULL	NULL	0	NULL	0.6-1300 U	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that 18 preparations contained antibiotic substances in an amount of 0.6-1300 U , equivalent to oxytetracycline units per 1 g. Most often antibiotics were present in preparations of the pectinase and protease group .
	manualset3
164323	5	412295	7	NULL	NULL	0	NULL	oxytetracycline 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that 18 preparations contained antibiotic substances in an amount of 0.6-1300 U , equivalent to oxytetracycline units per 1 g. Most often antibiotics were present in preparations of the pectinase and protease group .
	manualset3
164324	6	412295	7	NULL	NULL	0	NULL	 units per 1 g	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that 18 preparations contained antibiotic substances in an amount of 0.6-1300 U , equivalent to oxytetracycline units per 1 g. Most often antibiotics were present in preparations of the pectinase and protease group .
	manualset3
164325	7	412295	7	NULL	NULL	0	NULL	antibiotics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that 18 preparations contained antibiotic substances in an amount of 0.6-1300 U , equivalent to oxytetracycline units per 1 g. Most often antibiotics were present in preparations of the pectinase and protease group .
	manualset3
164326	8	412295	7	NULL	NULL	0	NULL	preparations	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that 18 preparations contained antibiotic substances in an amount of 0.6-1300 U , equivalent to oxytetracycline units per 1 g. Most often antibiotics were present in preparations of the pectinase and protease group .
	manualset3
164327	9	412295	7	NULL	NULL	0	NULL	 pectinase group	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that 18 preparations contained antibiotic substances in an amount of 0.6-1300 U , equivalent to oxytetracycline units per 1 g. Most often antibiotics were present in preparations of the pectinase and protease group .
	manualset3
164328	10	412295	7	NULL	NULL	0	NULL	protease group 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that 18 preparations contained antibiotic substances in an amount of 0.6-1300 U , equivalent to oxytetracycline units per 1 g. Most often antibiotics were present in preparations of the pectinase and protease group .
	manualset3
164329	1	412296	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed that 24h was adequate to obtain a significant response of the mites and that the soil properties tested ( moisture , pH , organic matter , and clay content ) had little influence on mite avoidance .
	manualset3
164330	2	412296	7	NULL	NULL	0	NULL	24h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that 24h was adequate to obtain a significant response of the mites and that the soil properties tested ( moisture , pH , organic matter , and clay content ) had little influence on mite avoidance .
	manualset3
164331	3	412296	7	NULL	NULL	NULL	NULL	response	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed that 24h was adequate to obtain a significant response of the mites and that the soil properties tested ( moisture , pH , organic matter , and clay content ) had little influence on mite avoidance .
	manualset3
164332	4	412296	7	NULL	NULL	0	NULL	mites	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that 24h was adequate to obtain a significant response of the mites and that the soil properties tested ( moisture , pH , organic matter , and clay content ) had little influence on mite avoidance .
	manualset3
164333	5	412296	7	NULL	NULL	0	NULL	soil properties	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that 24h was adequate to obtain a significant response of the mites and that the soil properties tested ( moisture , pH , organic matter , and clay content ) had little influence on mite avoidance .
	manualset3
164334	6	412296	7	NULL	NULL	NULL	NULL	moisture	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed that 24h was adequate to obtain a significant response of the mites and that the soil properties tested ( moisture , pH , organic matter , and clay content ) had little influence on mite avoidance .
	manualset3
164335	7	412296	7	NULL	NULL	0	NULL	pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that 24h was adequate to obtain a significant response of the mites and that the soil properties tested ( moisture , pH , organic matter , and clay content ) had little influence on mite avoidance .
	manualset3
164336	8	412296	7	NULL	NULL	0	NULL	organic matter	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that 24h was adequate to obtain a significant response of the mites and that the soil properties tested ( moisture , pH , organic matter , and clay content ) had little influence on mite avoidance .
	manualset3
164337	9	412296	7	NULL	NULL	0	NULL	clay content 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that 24h was adequate to obtain a significant response of the mites and that the soil properties tested ( moisture , pH , organic matter , and clay content ) had little influence on mite avoidance .
	manualset3
164338	10	412296	7	NULL	NULL	0	NULL	mite	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that 24h was adequate to obtain a significant response of the mites and that the soil properties tested ( moisture , pH , organic matter , and clay content ) had little influence on mite avoidance .
	manualset3
164339	11	412296	7	NULL	NULL	0	NULL	avoidance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that 24h was adequate to obtain a significant response of the mites and that the soil properties tested ( moisture , pH , organic matter , and clay content ) had little influence on mite avoidance .
	manualset3
164340	1	412297	7	NULL	NULL	0	NULL	PAEs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that PAEs could significantly reduce embryo hatchability , increase developmental malformations , and suppress the metamorphosis of abalone larvae .
	manualset3
164341	2	412297	7	NULL	NULL	0	NULL	embryo hatchability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that PAEs could significantly reduce embryo hatchability , increase developmental malformations , and suppress the metamorphosis of abalone larvae .
	manualset3
164342	3	412297	7	NULL	NULL	0	NULL	increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that PAEs could significantly reduce embryo hatchability , increase developmental malformations , and suppress the metamorphosis of abalone larvae .
	manualset3
164343	4	412297	7	NULL	NULL	0	NULL	developmental malformations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that PAEs could significantly reduce embryo hatchability , increase developmental malformations , and suppress the metamorphosis of abalone larvae .
	manualset3
164345	6	412297	7	NULL	NULL	0	NULL	metamorphosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that PAEs could significantly reduce embryo hatchability , increase developmental malformations , and suppress the metamorphosis of abalone larvae .
	manualset3
164346	7	412297	7	NULL	NULL	0	NULL	abalone larvae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that PAEs could significantly reduce embryo hatchability , increase developmental malformations , and suppress the metamorphosis of abalone larvae .
	manualset3
165220	8	412297	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that PAEs could significantly reduce embryo hatchability , increase developmental malformations , and suppress the metamorphosis of abalone larvae .
	manualset3
164347	1	412298	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed that at 30 min of polymerization , 10 nM , 30 nM and 30 microM of E ( 2 ) inhibited microtubule assembly by -70 % , -94 % , and -92 % , respectively ( p & lt ; 0.01 ) , while T at the same three concentrations stimulated it by +83 % , +66 % , and +121 % , respectively ( p & lt ; 0.05 ) .
	manualset3
164348	2	412298	7	NULL	NULL	0	NULL	 30 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that at 30 min of polymerization , 10 nM , 30 nM and 30 microM of E ( 2 ) inhibited microtubule assembly by -70 % , -94 % , and -92 % , respectively ( p & lt ; 0.01 ) , while T at the same three concentrations stimulated it by +83 % , +66 % , and +121 % , respectively ( p & lt ; 0.05 ) .
	manualset3
164349	3	412298	7	NULL	NULL	NULL	NULL	polymerization	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed that at 30 min of polymerization , 10 nM , 30 nM and 30 microM of E ( 2 ) inhibited microtubule assembly by -70 % , -94 % , and -92 % , respectively ( p & lt ; 0.01 ) , while T at the same three concentrations stimulated it by +83 % , +66 % , and +121 % , respectively ( p & lt ; 0.05 ) .
	manualset3
164350	4	412298	7	NULL	NULL	0	NULL	10 nM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that at 30 min of polymerization , 10 nM , 30 nM and 30 microM of E ( 2 ) inhibited microtubule assembly by -70 % , -94 % , and -92 % , respectively ( p & lt ; 0.01 ) , while T at the same three concentrations stimulated it by +83 % , +66 % , and +121 % , respectively ( p & lt ; 0.05 ) .
	manualset3
164351	5	412298	7	NULL	NULL	0	NULL	30 nM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that at 30 min of polymerization , 10 nM , 30 nM and 30 microM of E ( 2 ) inhibited microtubule assembly by -70 % , -94 % , and -92 % , respectively ( p & lt ; 0.01 ) , while T at the same three concentrations stimulated it by +83 % , +66 % , and +121 % , respectively ( p & lt ; 0.05 ) .
	manualset3
164352	6	412298	7	NULL	NULL	NULL	NULL	30 microM	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed that at 30 min of polymerization , 10 nM , 30 nM and 30 microM of E ( 2 ) inhibited microtubule assembly by -70 % , -94 % , and -92 % , respectively ( p & lt ; 0.01 ) , while T at the same three concentrations stimulated it by +83 % , +66 % , and +121 % , respectively ( p & lt ; 0.05 ) .
	manualset3
164353	7	412298	7	NULL	NULL	NULL	NULL	E ( 2 )	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed that at 30 min of polymerization , 10 nM , 30 nM and 30 microM of E ( 2 ) inhibited microtubule assembly by -70 % , -94 % , and -92 % , respectively ( p & lt ; 0.01 ) , while T at the same three concentrations stimulated it by +83 % , +66 % , and +121 % , respectively ( p & lt ; 0.05 ) .
	manualset3
164354	8	412298	7	NULL	NULL	0	NULL	microtubule assembly	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that at 30 min of polymerization , 10 nM , 30 nM and 30 microM of E ( 2 ) inhibited microtubule assembly by -70 % , -94 % , and -92 % , respectively ( p & lt ; 0.01 ) , while T at the same three concentrations stimulated it by +83 % , +66 % , and +121 % , respectively ( p & lt ; 0.05 ) .
	manualset3
164355	9	412298	7	NULL	NULL	0	NULL	-70 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that at 30 min of polymerization , 10 nM , 30 nM and 30 microM of E ( 2 ) inhibited microtubule assembly by -70 % , -94 % , and -92 % , respectively ( p & lt ; 0.01 ) , while T at the same three concentrations stimulated it by +83 % , +66 % , and +121 % , respectively ( p & lt ; 0.05 ) .
	manualset3
164356	10	412298	7	NULL	NULL	0	NULL	-94 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that at 30 min of polymerization , 10 nM , 30 nM and 30 microM of E ( 2 ) inhibited microtubule assembly by -70 % , -94 % , and -92 % , respectively ( p & lt ; 0.01 ) , while T at the same three concentrations stimulated it by +83 % , +66 % , and +121 % , respectively ( p & lt ; 0.05 ) .
	manualset3
164357	11	412298	7	NULL	NULL	0	NULL	-92 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that at 30 min of polymerization , 10 nM , 30 nM and 30 microM of E ( 2 ) inhibited microtubule assembly by -70 % , -94 % , and -92 % , respectively ( p & lt ; 0.01 ) , while T at the same three concentrations stimulated it by +83 % , +66 % , and +121 % , respectively ( p & lt ; 0.05 ) .
	manualset3
164358	12	412298	7	NULL	NULL	0	NULL	p & lt ; 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that at 30 min of polymerization , 10 nM , 30 nM and 30 microM of E ( 2 ) inhibited microtubule assembly by -70 % , -94 % , and -92 % , respectively ( p & lt ; 0.01 ) , while T at the same three concentrations stimulated it by +83 % , +66 % , and +121 % , respectively ( p & lt ; 0.05 ) .
	manualset3
164359	13	412298	7	NULL	NULL	0	NULL	T 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that at 30 min of polymerization , 10 nM , 30 nM and 30 microM of E ( 2 ) inhibited microtubule assembly by -70 % , -94 % , and -92 % , respectively ( p & lt ; 0.01 ) , while T at the same three concentrations stimulated it by +83 % , +66 % , and +121 % , respectively ( p & lt ; 0.05 ) .
	manualset3
164360	14	412298	7	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that at 30 min of polymerization , 10 nM , 30 nM and 30 microM of E ( 2 ) inhibited microtubule assembly by -70 % , -94 % , and -92 % , respectively ( p & lt ; 0.01 ) , while T at the same three concentrations stimulated it by +83 % , +66 % , and +121 % , respectively ( p & lt ; 0.05 ) .
	manualset3
164361	15	412298	7	NULL	NULL	0	NULL	concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that at 30 min of polymerization , 10 nM , 30 nM and 30 microM of E ( 2 ) inhibited microtubule assembly by -70 % , -94 % , and -92 % , respectively ( p & lt ; 0.01 ) , while T at the same three concentrations stimulated it by +83 % , +66 % , and +121 % , respectively ( p & lt ; 0.05 ) .
	manualset3
164362	16	412298	7	NULL	NULL	0	NULL	+83 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that at 30 min of polymerization , 10 nM , 30 nM and 30 microM of E ( 2 ) inhibited microtubule assembly by -70 % , -94 % , and -92 % , respectively ( p & lt ; 0.01 ) , while T at the same three concentrations stimulated it by +83 % , +66 % , and +121 % , respectively ( p & lt ; 0.05 ) .
	manualset3
164363	17	412298	7	NULL	NULL	0	NULL	+66 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that at 30 min of polymerization , 10 nM , 30 nM and 30 microM of E ( 2 ) inhibited microtubule assembly by -70 % , -94 % , and -92 % , respectively ( p & lt ; 0.01 ) , while T at the same three concentrations stimulated it by +83 % , +66 % , and +121 % , respectively ( p & lt ; 0.05 ) .
	manualset3
164364	18	412298	7	NULL	NULL	0	NULL	+121 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that at 30 min of polymerization , 10 nM , 30 nM and 30 microM of E ( 2 ) inhibited microtubule assembly by -70 % , -94 % , and -92 % , respectively ( p & lt ; 0.01 ) , while T at the same three concentrations stimulated it by +83 % , +66 % , and +121 % , respectively ( p & lt ; 0.05 ) .
	manualset3
164365	19	412298	7	NULL	NULL	0	NULL	 p & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that at 30 min of polymerization , 10 nM , 30 nM and 30 microM of E ( 2 ) inhibited microtubule assembly by -70 % , -94 % , and -92 % , respectively ( p & lt ; 0.01 ) , while T at the same three concentrations stimulated it by +83 % , +66 % , and +121 % , respectively ( p & lt ; 0.05 ) .
	manualset3
164366	1	412299	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed that benactyzine , caramiphen , and trihexyphenidyl reduced rats ' innate preference for novelty , whereas biperiden and procyclidine did not .
	manualset3
164367	2	412299	7	NULL	NULL	0	NULL	benactyzine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that benactyzine , caramiphen , and trihexyphenidyl reduced rats ' innate preference for novelty , whereas biperiden and procyclidine did not .
	manualset3
164368	3	412299	7	NULL	NULL	0	NULL	caramiphen	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that benactyzine , caramiphen , and trihexyphenidyl reduced rats ' innate preference for novelty , whereas biperiden and procyclidine did not .
	manualset3
164369	4	412299	7	NULL	NULL	0	NULL	trihexyphenidyl reduced rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that benactyzine , caramiphen , and trihexyphenidyl reduced rats ' innate preference for novelty , whereas biperiden and procyclidine did not .
	manualset3
164370	5	412299	7	NULL	NULL	0	NULL	innate preference	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that benactyzine , caramiphen , and trihexyphenidyl reduced rats ' innate preference for novelty , whereas biperiden and procyclidine did not .
	manualset3
164371	6	412299	7	NULL	NULL	0	NULL	novelty	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that benactyzine , caramiphen , and trihexyphenidyl reduced rats ' innate preference for novelty , whereas biperiden and procyclidine did not .
	manualset3
164372	7	412299	7	NULL	NULL	0	NULL	biperiden	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that benactyzine , caramiphen , and trihexyphenidyl reduced rats ' innate preference for novelty , whereas biperiden and procyclidine did not .
	manualset3
164373	8	412299	7	NULL	NULL	0	NULL	procyclidine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that benactyzine , caramiphen , and trihexyphenidyl reduced rats ' innate preference for novelty , whereas biperiden and procyclidine did not .
	manualset3
164374	1	412300	7	NULL	NULL	0	NULL	Acceptable precision 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Acceptable precision and accuracy ( + / -20 % deviation for LLOQ standard and + / -15 % deviation for other standards from the respective nominal concentration ) were obtained for concentrations over the standard curve ranges .
	manualset3
164375	2	412300	7	NULL	NULL	0	NULL	 accuracy 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Acceptable precision and accuracy ( + / -20 % deviation for LLOQ standard and + / -15 % deviation for other standards from the respective nominal concentration ) were obtained for concentrations over the standard curve ranges .
	manualset3
164376	3	412300	7	NULL	NULL	0	NULL	+ / -20 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Acceptable precision and accuracy ( + / -20 % deviation for LLOQ standard and + / -15 % deviation for other standards from the respective nominal concentration ) were obtained for concentrations over the standard curve ranges .
	manualset3
164377	4	412300	7	NULL	NULL	0	NULL	LLOQ standard	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Acceptable precision and accuracy ( + / -20 % deviation for LLOQ standard and + / -15 % deviation for other standards from the respective nominal concentration ) were obtained for concentrations over the standard curve ranges .
	manualset3
164378	5	412300	7	NULL	NULL	0	NULL	 + / -15 % deviation	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Acceptable precision and accuracy ( + / -20 % deviation for LLOQ standard and + / -15 % deviation for other standards from the respective nominal concentration ) were obtained for concentrations over the standard curve ranges .
	manualset3
164379	6	412300	7	NULL	NULL	0	NULL	standards	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Acceptable precision and accuracy ( + / -20 % deviation for LLOQ standard and + / -15 % deviation for other standards from the respective nominal concentration ) were obtained for concentrations over the standard curve ranges .
	manualset3
164380	7	412300	7	NULL	NULL	0	NULL	concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Acceptable precision and accuracy ( + / -20 % deviation for LLOQ standard and + / -15 % deviation for other standards from the respective nominal concentration ) were obtained for concentrations over the standard curve ranges .
	manualset3
164381	9	412300	7	NULL	NULL	NULL	NULL	standard curve ranges	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Acceptable precision and accuracy ( + / -20 % deviation for LLOQ standard and + / -15 % deviation for other standards from the respective nominal concentration ) were obtained for concentrations over the standard curve ranges .
	manualset3
164382	8	412300	7	NULL	NULL	0	NULL	concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Acceptable precision and accuracy ( + / -20 % deviation for LLOQ standard and + / -15 % deviation for other standards from the respective nominal concentration ) were obtained for concentrations over the standard curve ranges .
	manualset3
164383	1	412301	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed that body weight and composition were marginally affected by Eq administration ( P & gt ; 0.05 ) .
	manualset3
164384	2	412301	7	NULL	NULL	0	NULL	body weight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that body weight and composition were marginally affected by Eq administration ( P & gt ; 0.05 ) .
	manualset3
164385	3	412301	7	NULL	NULL	0	NULL	composition	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that body weight and composition were marginally affected by Eq administration ( P & gt ; 0.05 ) .
	manualset3
164386	4	412301	7	NULL	NULL	0	NULL	Eq administration 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that body weight and composition were marginally affected by Eq administration ( P & gt ; 0.05 ) .
	manualset3
164387	5	412301	7	NULL	NULL	0	NULL	P & gt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that body weight and composition were marginally affected by Eq administration ( P & gt ; 0.05 ) .
	manualset3
164388	1	412302	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that calcium diffusion was observed , in the first 16 days , in all situations in which there was Ca ( OH ) 2 paste inside the root canals .
	manualset3
164389	2	412302	7	NULL	NULL	0	NULL	calcium diffusion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that calcium diffusion was observed , in the first 16 days , in all situations in which there was Ca ( OH ) 2 paste inside the root canals .
	manualset3
164390	3	412302	7	NULL	NULL	0	NULL	first 16 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that calcium diffusion was observed , in the first 16 days , in all situations in which there was Ca ( OH ) 2 paste inside the root canals .
	manualset3
164391	4	412302	7	NULL	NULL	NULL	NULL	Ca ( OH ) 2 paste	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed that calcium diffusion was observed , in the first 16 days , in all situations in which there was Ca ( OH ) 2 paste inside the root canals .
	manualset3
164392	5	412302	7	NULL	NULL	0	NULL	 root canals	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that calcium diffusion was observed , in the first 16 days , in all situations in which there was Ca ( OH ) 2 paste inside the root canals .
	manualset3
164393	1	412303	7	NULL	NULL	0	NULL	results	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that high expression of c-Met accompanied with over-expression of SMYD3 .
	manualset3
164394	2	412303	7	NULL	NULL	0	NULL	high expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that high expression of c-Met accompanied with over-expression of SMYD3 .
	manualset3
164395	3	412303	7	NULL	NULL	0	NULL	c-Met	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that high expression of c-Met accompanied with over-expression of SMYD3 .
	manualset3
164396	4	412303	7	NULL	NULL	0	NULL	 over-expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that high expression of c-Met accompanied with over-expression of SMYD3 .
	manualset3
164397	5	412303	7	NULL	NULL	0	NULL	SMYD3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that high expression of c-Met accompanied with over-expression of SMYD3 .
	manualset3
164398	1	412304	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed that in ewes : 1 ) the regular cadmium intestinal intake negatively influences all reproductive parameters ; 2 ) cadmium is particularly accumulated in kidney and liver , but also in mammary gland , although at a distinctly lower level ; 3 ) chronic administration does not increase cadmium placental transfer in lactating pregnant subjects .
	manualset3
164399	2	412304	7	NULL	NULL	NULL	NULL	ewes	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed that in ewes : 1 ) the regular cadmium intestinal intake negatively influences all reproductive parameters ; 2 ) cadmium is particularly accumulated in kidney and liver , but also in mammary gland , although at a distinctly lower level ; 3 ) chronic administration does not increase cadmium placental transfer in lactating pregnant subjects .
	manualset3
164400	3	412304	7	NULL	NULL	0	NULL	cadmium 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that in ewes : 1 ) the regular cadmium intestinal intake negatively influences all reproductive parameters ; 2 ) cadmium is particularly accumulated in kidney and liver , but also in mammary gland , although at a distinctly lower level ; 3 ) chronic administration does not increase cadmium placental transfer in lactating pregnant subjects .
	manualset3
164401	4	412304	7	NULL	NULL	0	NULL	 intestinal intake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that in ewes : 1 ) the regular cadmium intestinal intake negatively influences all reproductive parameters ; 2 ) cadmium is particularly accumulated in kidney and liver , but also in mammary gland , although at a distinctly lower level ; 3 ) chronic administration does not increase cadmium placental transfer in lactating pregnant subjects .
	manualset3
164402	5	412304	7	NULL	NULL	NULL	NULL	reproductive parameters	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed that in ewes : 1 ) the regular cadmium intestinal intake negatively influences all reproductive parameters ; 2 ) cadmium is particularly accumulated in kidney and liver , but also in mammary gland , although at a distinctly lower level ; 3 ) chronic administration does not increase cadmium placental transfer in lactating pregnant subjects .
	manualset3
164403	6	412304	7	NULL	NULL	0	NULL	cadmium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that in ewes : 1 ) the regular cadmium intestinal intake negatively influences all reproductive parameters ; 2 ) cadmium is particularly accumulated in kidney and liver , but also in mammary gland , although at a distinctly lower level ; 3 ) chronic administration does not increase cadmium placental transfer in lactating pregnant subjects .
	manualset3
164404	7	412304	7	NULL	NULL	0	NULL	kidney	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that in ewes : 1 ) the regular cadmium intestinal intake negatively influences all reproductive parameters ; 2 ) cadmium is particularly accumulated in kidney and liver , but also in mammary gland , although at a distinctly lower level ; 3 ) chronic administration does not increase cadmium placental transfer in lactating pregnant subjects .
	manualset3
164405	8	412304	7	NULL	NULL	0	NULL	liver 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that in ewes : 1 ) the regular cadmium intestinal intake negatively influences all reproductive parameters ; 2 ) cadmium is particularly accumulated in kidney and liver , but also in mammary gland , although at a distinctly lower level ; 3 ) chronic administration does not increase cadmium placental transfer in lactating pregnant subjects .
	manualset3
164406	9	412304	7	NULL	NULL	0	NULL	mammary gland	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that in ewes : 1 ) the regular cadmium intestinal intake negatively influences all reproductive parameters ; 2 ) cadmium is particularly accumulated in kidney and liver , but also in mammary gland , although at a distinctly lower level ; 3 ) chronic administration does not increase cadmium placental transfer in lactating pregnant subjects .
	manualset3
164407	10	412304	7	NULL	NULL	0	NULL	lower level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that in ewes : 1 ) the regular cadmium intestinal intake negatively influences all reproductive parameters ; 2 ) cadmium is particularly accumulated in kidney and liver , but also in mammary gland , although at a distinctly lower level ; 3 ) chronic administration does not increase cadmium placental transfer in lactating pregnant subjects .
	manualset3
164408	11	412304	7	NULL	NULL	0	NULL	chronic administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that in ewes : 1 ) the regular cadmium intestinal intake negatively influences all reproductive parameters ; 2 ) cadmium is particularly accumulated in kidney and liver , but also in mammary gland , although at a distinctly lower level ; 3 ) chronic administration does not increase cadmium placental transfer in lactating pregnant subjects .
	manualset3
164409	12	412304	7	NULL	NULL	0	NULL	cadmium placental transfer	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that in ewes : 1 ) the regular cadmium intestinal intake negatively influences all reproductive parameters ; 2 ) cadmium is particularly accumulated in kidney and liver , but also in mammary gland , although at a distinctly lower level ; 3 ) chronic administration does not increase cadmium placental transfer in lactating pregnant subjects .
	manualset3
164410	13	412304	7	NULL	NULL	0	NULL	lactating pregnant subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that in ewes : 1 ) the regular cadmium intestinal intake negatively influences all reproductive parameters ; 2 ) cadmium is particularly accumulated in kidney and liver , but also in mammary gland , although at a distinctly lower level ; 3 ) chronic administration does not increase cadmium placental transfer in lactating pregnant subjects .
	manualset3
164411	1	412305	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed that streptozotocin-induced diabetic rats showed insulin-resistance through alterations in the kinetics of insulin receptor binding .
	manualset3
164412	2	412305	7	NULL	NULL	0	NULL	streptozotocin-induced diabetic rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that streptozotocin-induced diabetic rats showed insulin-resistance through alterations in the kinetics of insulin receptor binding .
	manualset3
164413	3	412305	7	NULL	NULL	0	NULL	insulin-resistance	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that streptozotocin-induced diabetic rats showed insulin-resistance through alterations in the kinetics of insulin receptor binding .
	manualset3
164414	4	412305	7	NULL	NULL	0	NULL	 alterations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that streptozotocin-induced diabetic rats showed insulin-resistance through alterations in the kinetics of insulin receptor binding .
	manualset3
164415	5	412305	7	NULL	NULL	0	NULL	kinetics	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that streptozotocin-induced diabetic rats showed insulin-resistance through alterations in the kinetics of insulin receptor binding .
	manualset3
164416	6	412305	7	NULL	NULL	0	NULL	 insulin receptor binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that streptozotocin-induced diabetic rats showed insulin-resistance through alterations in the kinetics of insulin receptor binding .
	manualset3
164417	1	412306	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed that the immediate increase in kidney weight due to inflammatory swelling was associated with simultaneous elevation of serum thromboxane and leukotriene levels .
	manualset3
164418	2	412306	7	NULL	NULL	NULL	NULL	increase	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed that the immediate increase in kidney weight due to inflammatory swelling was associated with simultaneous elevation of serum thromboxane and leukotriene levels .
	manualset3
164419	3	412306	7	NULL	NULL	0	NULL	kidney weight	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that the immediate increase in kidney weight due to inflammatory swelling was associated with simultaneous elevation of serum thromboxane and leukotriene levels .
	manualset3
164420	4	412306	7	NULL	NULL	0	NULL	inflammatory swelling	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that the immediate increase in kidney weight due to inflammatory swelling was associated with simultaneous elevation of serum thromboxane and leukotriene levels .
	manualset3
164421	5	412306	7	NULL	NULL	0	NULL	elevation	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that the immediate increase in kidney weight due to inflammatory swelling was associated with simultaneous elevation of serum thromboxane and leukotriene levels .
	manualset3
164422	6	412306	7	NULL	NULL	NULL	NULL	serum thromboxane levels	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed that the immediate increase in kidney weight due to inflammatory swelling was associated with simultaneous elevation of serum thromboxane and leukotriene levels .
	manualset3
164423	7	412306	7	NULL	NULL	0	NULL	leukotriene levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that the immediate increase in kidney weight due to inflammatory swelling was associated with simultaneous elevation of serum thromboxane and leukotriene levels .
	manualset3
164424	1	412307	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that the interincisal dimension is a fairly reliable measure of mandibular mobility even when the length of the mandible is altered with surgery .
	manualset3
164425	2	412307	7	NULL	NULL	0	NULL	interincisal dimension	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that the interincisal dimension is a fairly reliable measure of mandibular mobility even when the length of the mandible is altered with surgery .
	manualset3
164426	3	412307	7	NULL	NULL	0	NULL	measure	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that the interincisal dimension is a fairly reliable measure of mandibular mobility even when the length of the mandible is altered with surgery .
	manualset3
164427	4	412307	7	NULL	NULL	0	NULL	mandibular mobility 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that the interincisal dimension is a fairly reliable measure of mandibular mobility even when the length of the mandible is altered with surgery .
	manualset3
164428	5	412307	7	NULL	NULL	0	NULL	length	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that the interincisal dimension is a fairly reliable measure of mandibular mobility even when the length of the mandible is altered with surgery .
	manualset3
164429	6	412307	7	NULL	NULL	0	NULL	mandible	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that the interincisal dimension is a fairly reliable measure of mandibular mobility even when the length of the mandible is altered with surgery .
	manualset3
164430	7	412307	7	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that the interincisal dimension is a fairly reliable measure of mandibular mobility even when the length of the mandible is altered with surgery .
	manualset3
164431	1	412308	7	NULL	NULL	0	NULL	 results	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that the synthesized gene and cloned gene were identical to the HBD4 gene sequence registered in GenBank and were successfully cloned into cloning vector pMD18-T and prokaryotic expression vector pGEX-4T-2 .
	manualset3
164432	2	412308	7	NULL	NULL	0	NULL	synthesized gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that the synthesized gene and cloned gene were identical to the HBD4 gene sequence registered in GenBank and were successfully cloned into cloning vector pMD18-T and prokaryotic expression vector pGEX-4T-2 .
	manualset3
164433	3	412308	7	NULL	NULL	0	NULL	 cloned gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that the synthesized gene and cloned gene were identical to the HBD4 gene sequence registered in GenBank and were successfully cloned into cloning vector pMD18-T and prokaryotic expression vector pGEX-4T-2 .
	manualset3
164434	4	412308	7	NULL	NULL	0	NULL	HBD4 gene sequence	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that the synthesized gene and cloned gene were identical to the HBD4 gene sequence registered in GenBank and were successfully cloned into cloning vector pMD18-T and prokaryotic expression vector pGEX-4T-2 .
	manualset3
164435	5	412308	7	NULL	NULL	0	NULL	GenBank	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that the synthesized gene and cloned gene were identical to the HBD4 gene sequence registered in GenBank and were successfully cloned into cloning vector pMD18-T and prokaryotic expression vector pGEX-4T-2 .
	manualset3
164436	6	412308	7	NULL	NULL	0	NULL	cloning vector pMD18-T 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that the synthesized gene and cloned gene were identical to the HBD4 gene sequence registered in GenBank and were successfully cloned into cloning vector pMD18-T and prokaryotic expression vector pGEX-4T-2 .
	manualset3
164437	7	412308	7	NULL	NULL	0	NULL	prokaryotic expression vector pGEX-4T-2	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that the synthesized gene and cloned gene were identical to the HBD4 gene sequence registered in GenBank and were successfully cloned into cloning vector pMD18-T and prokaryotic expression vector pGEX-4T-2 .
	manualset3
164438	1	412309	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed that the treatment of SNE significantly lowered the CCl4-induced serum levels of hepatic enzyme markers ( GOT , GPT , ALP , and total bilirubin ) , superoxide and hydroxyl radical .
	manualset3
164439	2	412309	7	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that the treatment of SNE significantly lowered the CCl4-induced serum levels of hepatic enzyme markers ( GOT , GPT , ALP , and total bilirubin ) , superoxide and hydroxyl radical .
	manualset3
164440	3	412309	7	NULL	NULL	0	NULL	SNE	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that the treatment of SNE significantly lowered the CCl4-induced serum levels of hepatic enzyme markers ( GOT , GPT , ALP , and total bilirubin ) , superoxide and hydroxyl radical .
	manualset3
164441	4	412309	7	NULL	NULL	0	NULL	CCl4-induced serum levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that the treatment of SNE significantly lowered the CCl4-induced serum levels of hepatic enzyme markers ( GOT , GPT , ALP , and total bilirubin ) , superoxide and hydroxyl radical .
	manualset3
164442	5	412309	7	NULL	NULL	0	NULL	hepatic enzyme markers 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that the treatment of SNE significantly lowered the CCl4-induced serum levels of hepatic enzyme markers ( GOT , GPT , ALP , and total bilirubin ) , superoxide and hydroxyl radical .
	manualset3
164443	6	412309	7	NULL	NULL	0	NULL	GOT	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that the treatment of SNE significantly lowered the CCl4-induced serum levels of hepatic enzyme markers ( GOT , GPT , ALP , and total bilirubin ) , superoxide and hydroxyl radical .
	manualset3
164444	7	412309	7	NULL	NULL	0	NULL	GPT	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that the treatment of SNE significantly lowered the CCl4-induced serum levels of hepatic enzyme markers ( GOT , GPT , ALP , and total bilirubin ) , superoxide and hydroxyl radical .
	manualset3
164445	8	412309	7	NULL	NULL	0	NULL	ALP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that the treatment of SNE significantly lowered the CCl4-induced serum levels of hepatic enzyme markers ( GOT , GPT , ALP , and total bilirubin ) , superoxide and hydroxyl radical .
	manualset3
164446	9	412309	7	NULL	NULL	0	NULL	total bilirubin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that the treatment of SNE significantly lowered the CCl4-induced serum levels of hepatic enzyme markers ( GOT , GPT , ALP , and total bilirubin ) , superoxide and hydroxyl radical .
	manualset3
164447	10	412309	7	NULL	NULL	0	NULL	superoxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that the treatment of SNE significantly lowered the CCl4-induced serum levels of hepatic enzyme markers ( GOT , GPT , ALP , and total bilirubin ) , superoxide and hydroxyl radical .
	manualset3
164448	11	412309	7	NULL	NULL	0	NULL	hydroxyl radical	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that the treatment of SNE significantly lowered the CCl4-induced serum levels of hepatic enzyme markers ( GOT , GPT , ALP , and total bilirubin ) , superoxide and hydroxyl radical .
	manualset3
164449	1	412310	7	NULL	NULL	0	NULL	Acceptance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acceptance of zidovudine ( AZT ) in early HIV disease : the role of health beliefs .
	manualset3
164450	2	412310	7	NULL	NULL	0	NULL	zidovudine ( AZT )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Acceptance of zidovudine ( AZT ) in early HIV disease : the role of health beliefs .
	manualset3
164451	3	412310	7	NULL	NULL	0	NULL	 early HIV disease	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acceptance of zidovudine ( AZT ) in early HIV disease : the role of health beliefs .
	manualset3
164452	4	412310	7	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Acceptance of zidovudine ( AZT ) in early HIV disease : the role of health beliefs .
	manualset3
164453	5	412310	7	NULL	NULL	0	NULL	health beliefs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acceptance of zidovudine ( AZT ) in early HIV disease : the role of health beliefs .
	manualset3
164454	1	412311	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results showed that treatment with L-NIL suppressed both NO production and iNOS activity but enhanced specific IgG2a , IFN-gamma levels , and increased cell proliferation following stimulation with A. actinomycetemcomitans LPS-stimulated cells .
	manualset3
164455	2	412311	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that treatment with L-NIL suppressed both NO production and iNOS activity but enhanced specific IgG2a , IFN-gamma levels , and increased cell proliferation following stimulation with A. actinomycetemcomitans LPS-stimulated cells .
	manualset3
164456	3	412311	7	NULL	NULL	0	NULL	L-NIL	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that treatment with L-NIL suppressed both NO production and iNOS activity but enhanced specific IgG2a , IFN-gamma levels , and increased cell proliferation following stimulation with A. actinomycetemcomitans LPS-stimulated cells .
	manualset3
164457	4	412311	7	NULL	NULL	0	NULL	NO production 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that treatment with L-NIL suppressed both NO production and iNOS activity but enhanced specific IgG2a , IFN-gamma levels , and increased cell proliferation following stimulation with A. actinomycetemcomitans LPS-stimulated cells .
	manualset3
164458	5	412311	7	NULL	NULL	0	NULL	 iNOS activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that treatment with L-NIL suppressed both NO production and iNOS activity but enhanced specific IgG2a , IFN-gamma levels , and increased cell proliferation following stimulation with A. actinomycetemcomitans LPS-stimulated cells .
	manualset3
164459	6	412311	7	NULL	NULL	0	NULL	IgG2a levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that treatment with L-NIL suppressed both NO production and iNOS activity but enhanced specific IgG2a , IFN-gamma levels , and increased cell proliferation following stimulation with A. actinomycetemcomitans LPS-stimulated cells .
	manualset3
164460	7	412311	7	NULL	NULL	0	NULL	IFN-gamma levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that treatment with L-NIL suppressed both NO production and iNOS activity but enhanced specific IgG2a , IFN-gamma levels , and increased cell proliferation following stimulation with A. actinomycetemcomitans LPS-stimulated cells .
	manualset3
164461	8	412311	7	NULL	NULL	0	NULL	cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that treatment with L-NIL suppressed both NO production and iNOS activity but enhanced specific IgG2a , IFN-gamma levels , and increased cell proliferation following stimulation with A. actinomycetemcomitans LPS-stimulated cells .
	manualset3
164462	9	412311	7	NULL	NULL	0	NULL	stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that treatment with L-NIL suppressed both NO production and iNOS activity but enhanced specific IgG2a , IFN-gamma levels , and increased cell proliferation following stimulation with A. actinomycetemcomitans LPS-stimulated cells .
	manualset3
164463	10	412311	7	NULL	NULL	0	NULL	 A. actinomycetemcomitans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that treatment with L-NIL suppressed both NO production and iNOS activity but enhanced specific IgG2a , IFN-gamma levels , and increased cell proliferation following stimulation with A. actinomycetemcomitans LPS-stimulated cells .
	manualset3
164464	11	412311	7	NULL	NULL	0	NULL	LPS-stimulated cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that treatment with L-NIL suppressed both NO production and iNOS activity but enhanced specific IgG2a , IFN-gamma levels , and increased cell proliferation following stimulation with A. actinomycetemcomitans LPS-stimulated cells .
	manualset3
165221	1	412312	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that with Amalgambond , there was significantly better sealing of the dentin tubules than with Copalite or unlined restorations ( P & lt ; 0.001 ) at all times tested .
	manualset3
165222	2	412312	7	NULL	NULL	0	NULL	Amalgambond 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that with Amalgambond , there was significantly better sealing of the dentin tubules than with Copalite or unlined restorations ( P & lt ; 0.001 ) at all times tested .
	manualset3
165223	3	412312	7	NULL	NULL	0	NULL	sealing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that with Amalgambond , there was significantly better sealing of the dentin tubules than with Copalite or unlined restorations ( P & lt ; 0.001 ) at all times tested .
	manualset3
165224	4	412312	7	NULL	NULL	0	NULL	dentin tubules	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that with Amalgambond , there was significantly better sealing of the dentin tubules than with Copalite or unlined restorations ( P & lt ; 0.001 ) at all times tested .
	manualset3
165225	5	412312	7	NULL	NULL	0	NULL	 Copalite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that with Amalgambond , there was significantly better sealing of the dentin tubules than with Copalite or unlined restorations ( P & lt ; 0.001 ) at all times tested .
	manualset3
165226	6	412312	7	NULL	NULL	0	NULL	unlined restorations	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that with Amalgambond , there was significantly better sealing of the dentin tubules than with Copalite or unlined restorations ( P & lt ; 0.001 ) at all times tested .
	manualset3
165227	7	412312	7	NULL	NULL	0	NULL	 P & lt ; 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that with Amalgambond , there was significantly better sealing of the dentin tubules than with Copalite or unlined restorations ( P & lt ; 0.001 ) at all times tested .
	manualset3
165228	8	412312	7	NULL	NULL	0	NULL	times 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The results showed that with Amalgambond , there was significantly better sealing of the dentin tubules than with Copalite or unlined restorations ( P & lt ; 0.001 ) at all times tested .
	manualset3
164465	1	412313	7	NULL	NULL	NULL	NULL	results 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results suggest ( 1 ) F1 and F2 to be equivalent exposure conditions and ( 2 ) the dominance of vestibular-auditory interactions , compared with visual-auditory ones .
	manualset3
164466	2	412313	7	NULL	NULL	0	NULL	 F1	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest ( 1 ) F1 and F2 to be equivalent exposure conditions and ( 2 ) the dominance of vestibular-auditory interactions , compared with visual-auditory ones .
	manualset3
164467	3	412313	7	NULL	NULL	0	NULL	F2	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest ( 1 ) F1 and F2 to be equivalent exposure conditions and ( 2 ) the dominance of vestibular-auditory interactions , compared with visual-auditory ones .
	manualset3
164468	4	412313	7	NULL	NULL	0	NULL	 conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest ( 1 ) F1 and F2 to be equivalent exposure conditions and ( 2 ) the dominance of vestibular-auditory interactions , compared with visual-auditory ones .
	manualset3
164469	5	412313	7	NULL	NULL	0	NULL	dominance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest ( 1 ) F1 and F2 to be equivalent exposure conditions and ( 2 ) the dominance of vestibular-auditory interactions , compared with visual-auditory ones .
	manualset3
164470	6	412313	7	NULL	NULL	0	NULL	vestibular-auditory interactions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest ( 1 ) F1 and F2 to be equivalent exposure conditions and ( 2 ) the dominance of vestibular-auditory interactions , compared with visual-auditory ones .
	manualset3
164471	7	412313	7	NULL	NULL	0	NULL	visual-auditory ones	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest ( 1 ) F1 and F2 to be equivalent exposure conditions and ( 2 ) the dominance of vestibular-auditory interactions , compared with visual-auditory ones .
	manualset3
164472	1	412314	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest a dose-related inhibitory effect of secretin on prolactin release in women .
	manualset3
164473	2	412314	7	NULL	NULL	0	NULL	dose-related inhibitory effect 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest a dose-related inhibitory effect of secretin on prolactin release in women .
	manualset3
164474	3	412314	7	NULL	NULL	0	NULL	secretin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest a dose-related inhibitory effect of secretin on prolactin release in women .
	manualset3
164475	4	412314	7	NULL	NULL	0	NULL	prolactin release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest a dose-related inhibitory effect of secretin on prolactin release in women .
	manualset3
164476	5	412314	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest a dose-related inhibitory effect of secretin on prolactin release in women .
	manualset3
164477	1	412315	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest a key role for L0 helix in KATP gating and together with previous findings from mutant KATP clarify why many patients with neonatal diabetes require high doses of sulfonylureas .
	manualset3
164478	2	412315	7	NULL	NULL	0	NULL	role 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest a key role for L0 helix in KATP gating and together with previous findings from mutant KATP clarify why many patients with neonatal diabetes require high doses of sulfonylureas .
	manualset3
164479	3	412315	7	NULL	NULL	0	NULL	L0 helix	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest a key role for L0 helix in KATP gating and together with previous findings from mutant KATP clarify why many patients with neonatal diabetes require high doses of sulfonylureas .
	manualset3
164480	4	412315	7	NULL	NULL	0	NULL	KATP gating	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest a key role for L0 helix in KATP gating and together with previous findings from mutant KATP clarify why many patients with neonatal diabetes require high doses of sulfonylureas .
	manualset3
164481	5	412315	7	NULL	NULL	0	NULL	 findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest a key role for L0 helix in KATP gating and together with previous findings from mutant KATP clarify why many patients with neonatal diabetes require high doses of sulfonylureas .
	manualset3
164482	6	412315	7	NULL	NULL	0	NULL	mutant KATP	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest a key role for L0 helix in KATP gating and together with previous findings from mutant KATP clarify why many patients with neonatal diabetes require high doses of sulfonylureas .
	manualset3
164483	7	412315	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest a key role for L0 helix in KATP gating and together with previous findings from mutant KATP clarify why many patients with neonatal diabetes require high doses of sulfonylureas .
	manualset3
164484	8	412315	7	NULL	NULL	0	NULL	neonatal diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest a key role for L0 helix in KATP gating and together with previous findings from mutant KATP clarify why many patients with neonatal diabetes require high doses of sulfonylureas .
	manualset3
164485	9	412315	7	NULL	NULL	0	NULL	high doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest a key role for L0 helix in KATP gating and together with previous findings from mutant KATP clarify why many patients with neonatal diabetes require high doses of sulfonylureas .
	manualset3
164486	10	412315	7	NULL	NULL	0	NULL	sulfonylureas	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest a key role for L0 helix in KATP gating and together with previous findings from mutant KATP clarify why many patients with neonatal diabetes require high doses of sulfonylureas .
	manualset3
164487	1	412316	7	NULL	NULL	0	NULL	results 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest a shift in the pro-oxidant/antioxidant balance in favor of lipid peroxidation .
	manualset3
164488	2	412316	7	NULL	NULL	NULL	NULL	shift 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results suggest a shift in the pro-oxidant/antioxidant balance in favor of lipid peroxidation .
	manualset3
164489	3	412316	7	NULL	NULL	NULL	NULL	 pro-oxidant/antioxidant balance	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results suggest a shift in the pro-oxidant/antioxidant balance in favor of lipid peroxidation .
	manualset3
164490	4	412316	7	NULL	NULL	0	NULL	 lipid peroxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest a shift in the pro-oxidant/antioxidant balance in favor of lipid peroxidation .
	manualset3
164491	1	412317	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest rapid passive extravascular diffusion of gadolinium ( Gd ) - DOTA in the interstitial space without intracellular penetration , followed by a rapid urinary excretion via glomerular filtration .
	manualset3
164492	2	412317	7	NULL	NULL	0	NULL	 rapid passive extravascular diffusion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest rapid passive extravascular diffusion of gadolinium ( Gd ) - DOTA in the interstitial space without intracellular penetration , followed by a rapid urinary excretion via glomerular filtration .
	manualset3
164493	3	412317	7	NULL	NULL	0	NULL	gadolinium ( Gd ) - DOTA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest rapid passive extravascular diffusion of gadolinium ( Gd ) - DOTA in the interstitial space without intracellular penetration , followed by a rapid urinary excretion via glomerular filtration .
	manualset3
164494	4	412317	7	NULL	NULL	0	NULL	interstitial space	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest rapid passive extravascular diffusion of gadolinium ( Gd ) - DOTA in the interstitial space without intracellular penetration , followed by a rapid urinary excretion via glomerular filtration .
	manualset3
164495	5	412317	7	NULL	NULL	0	NULL	intracellular penetration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest rapid passive extravascular diffusion of gadolinium ( Gd ) - DOTA in the interstitial space without intracellular penetration , followed by a rapid urinary excretion via glomerular filtration .
	manualset3
164496	6	412317	7	NULL	NULL	0	NULL	urinary excretion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest rapid passive extravascular diffusion of gadolinium ( Gd ) - DOTA in the interstitial space without intracellular penetration , followed by a rapid urinary excretion via glomerular filtration .
	manualset3
164497	7	412317	7	NULL	NULL	0	NULL	glomerular filtration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest rapid passive extravascular diffusion of gadolinium ( Gd ) - DOTA in the interstitial space without intracellular penetration , followed by a rapid urinary excretion via glomerular filtration .
	manualset3
164498	1	412318	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results suggest that Ach induced coronary vasoconstriction in CBS - / + mice and this vasoconstriction was ameliorated by FA treatment .
	manualset3
164499	2	412318	7	NULL	NULL	0	NULL	Ach 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that Ach induced coronary vasoconstriction in CBS - / + mice and this vasoconstriction was ameliorated by FA treatment .
	manualset3
164500	3	412318	7	NULL	NULL	0	NULL	coronary vasoconstriction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that Ach induced coronary vasoconstriction in CBS - / + mice and this vasoconstriction was ameliorated by FA treatment .
	manualset3
164501	4	412318	7	NULL	NULL	0	NULL	CBS - / + mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that Ach induced coronary vasoconstriction in CBS - / + mice and this vasoconstriction was ameliorated by FA treatment .
	manualset3
164502	5	412318	7	NULL	NULL	0	NULL	vasoconstriction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that Ach induced coronary vasoconstriction in CBS - / + mice and this vasoconstriction was ameliorated by FA treatment .
	manualset3
164503	6	412318	7	NULL	NULL	NULL	NULL	FA treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results suggest that Ach induced coronary vasoconstriction in CBS - / + mice and this vasoconstriction was ameliorated by FA treatment .
	manualset3
164505	1	412319	7	NULL	NULL	0	NULL	CCK-5-8	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that CCK-5-8 can amplify the arousal enhancement elicited by novelty through a central mechanism .
	manualset3
164506	2	412319	7	NULL	NULL	0	NULL	arousal enhancement	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that CCK-5-8 can amplify the arousal enhancement elicited by novelty through a central mechanism .
	manualset3
164507	3	412319	7	NULL	NULL	NULL	NULL	novelty	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results suggest that CCK-5-8 can amplify the arousal enhancement elicited by novelty through a central mechanism .
	manualset3
164508	4	412319	7	NULL	NULL	0	NULL	 central mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that CCK-5-8 can amplify the arousal enhancement elicited by novelty through a central mechanism .
	manualset3
164509	1	412320	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results suggest that CD4 mimicry by 16D7 is based on a conformational epitope and L2 is only one of the HP2/6-specific contact points of 16D7 .
	manualset3
164510	2	412320	7	NULL	NULL	0	NULL	CD4 mimicry	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that CD4 mimicry by 16D7 is based on a conformational epitope and L2 is only one of the HP2/6-specific contact points of 16D7 .
	manualset3
164511	3	412320	7	NULL	NULL	0	NULL	16D7	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that CD4 mimicry by 16D7 is based on a conformational epitope and L2 is only one of the HP2/6-specific contact points of 16D7 .
	manualset3
164512	4	412320	7	NULL	NULL	0	NULL	 conformational epitope	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that CD4 mimicry by 16D7 is based on a conformational epitope and L2 is only one of the HP2/6-specific contact points of 16D7 .
	manualset3
164513	5	412320	7	NULL	NULL	0	NULL	L2	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that CD4 mimicry by 16D7 is based on a conformational epitope and L2 is only one of the HP2/6-specific contact points of 16D7 .
	manualset3
164514	6	412320	7	NULL	NULL	0	NULL	HP2/6-specific contact points	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that CD4 mimicry by 16D7 is based on a conformational epitope and L2 is only one of the HP2/6-specific contact points of 16D7 .
	manualset3
164515	7	412320	7	NULL	NULL	0	NULL	16D7	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that CD4 mimicry by 16D7 is based on a conformational epitope and L2 is only one of the HP2/6-specific contact points of 16D7 .
	manualset3
164516	1	412321	7	NULL	NULL	NULL	NULL	results 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results suggest that a soybean oil-based diet can alter physiological mechanisms which mediate these indices of pain perception and thermoregulation .
	manualset3
164517	2	412321	7	NULL	NULL	0	NULL	soybean oil-based diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that a soybean oil-based diet can alter physiological mechanisms which mediate these indices of pain perception and thermoregulation .
	manualset3
164518	3	412321	7	NULL	NULL	0	NULL	physiological mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that a soybean oil-based diet can alter physiological mechanisms which mediate these indices of pain perception and thermoregulation .
	manualset3
164519	4	412321	7	NULL	NULL	0	NULL	 indices	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that a soybean oil-based diet can alter physiological mechanisms which mediate these indices of pain perception and thermoregulation .
	manualset3
164520	5	412321	7	NULL	NULL	0	NULL	pain perception	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that a soybean oil-based diet can alter physiological mechanisms which mediate these indices of pain perception and thermoregulation .
	manualset3
164521	6	412321	7	NULL	NULL	0	NULL	thermoregulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that a soybean oil-based diet can alter physiological mechanisms which mediate these indices of pain perception and thermoregulation .
	manualset3
164522	1	412322	7	NULL	NULL	NULL	NULL	results 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results suggest that anxiety is unlikely to be invariably associated with increased noradrenergic transmission , in the frontal cortex at least .
	manualset3
164523	2	412322	7	NULL	NULL	0	NULL	anxiety	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that anxiety is unlikely to be invariably associated with increased noradrenergic transmission , in the frontal cortex at least .
	manualset3
164524	3	412322	7	NULL	NULL	0	NULL	increased noradrenergic transmission	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that anxiety is unlikely to be invariably associated with increased noradrenergic transmission , in the frontal cortex at least .
	manualset3
164525	4	412322	7	NULL	NULL	0	NULL	frontal cortex 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that anxiety is unlikely to be invariably associated with increased noradrenergic transmission , in the frontal cortex at least .
	manualset3
164526	1	412323	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results suggest that apart from PSA , elevated antigen levels in elderly subjects are related to the ageing process itself rather than to occult pathology .
	manualset3
164527	2	412323	7	NULL	NULL	0	NULL	PSA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that apart from PSA , elevated antigen levels in elderly subjects are related to the ageing process itself rather than to occult pathology .
	manualset3
164528	3	412323	7	NULL	NULL	0	NULL	antigen levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that apart from PSA , elevated antigen levels in elderly subjects are related to the ageing process itself rather than to occult pathology .
	manualset3
164529	4	412323	7	NULL	NULL	0	NULL	elderly subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that apart from PSA , elevated antigen levels in elderly subjects are related to the ageing process itself rather than to occult pathology .
	manualset3
164530	5	412323	7	NULL	NULL	0	NULL	ageing process	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that apart from PSA , elevated antigen levels in elderly subjects are related to the ageing process itself rather than to occult pathology .
	manualset3
164531	6	412323	7	NULL	NULL	0	NULL	occult pathology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that apart from PSA , elevated antigen levels in elderly subjects are related to the ageing process itself rather than to occult pathology .
	manualset3
164532	1	412324	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results suggest that auditory stimuli produce more robust P300 components than visual stimuli in passive task situations .
	manualset3
164533	2	412324	7	NULL	NULL	0	NULL	 auditory stimuli	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that auditory stimuli produce more robust P300 components than visual stimuli in passive task situations .
	manualset3
164534	3	412324	7	NULL	NULL	NULL	NULL	P300 components	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results suggest that auditory stimuli produce more robust P300 components than visual stimuli in passive task situations .
	manualset3
164535	4	412324	7	NULL	NULL	0	NULL	 visual stimuli	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that auditory stimuli produce more robust P300 components than visual stimuli in passive task situations .
	manualset3
164536	5	412324	7	NULL	NULL	0	NULL	passive task situations	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that auditory stimuli produce more robust P300 components than visual stimuli in passive task situations .
	manualset3
164537	1	412325	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results suggest that fluctuations in the ethanol concentration are caused by variation in the ventilation/perfusion ratio of regions of the lung supplying the expirate , and that breath with ethanol in equilibrium with the plasma is not routinely obtained , especially at the end of a maximal expiration .
	manualset3
164538	2	412325	7	NULL	NULL	0	NULL	fluctuations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that fluctuations in the ethanol concentration are caused by variation in the ventilation/perfusion ratio of regions of the lung supplying the expirate , and that breath with ethanol in equilibrium with the plasma is not routinely obtained , especially at the end of a maximal expiration .
	manualset3
164539	3	412325	7	NULL	NULL	0	NULL	ethanol concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that fluctuations in the ethanol concentration are caused by variation in the ventilation/perfusion ratio of regions of the lung supplying the expirate , and that breath with ethanol in equilibrium with the plasma is not routinely obtained , especially at the end of a maximal expiration .
	manualset3
164540	4	412325	7	NULL	NULL	0	NULL	 variation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that fluctuations in the ethanol concentration are caused by variation in the ventilation/perfusion ratio of regions of the lung supplying the expirate , and that breath with ethanol in equilibrium with the plasma is not routinely obtained , especially at the end of a maximal expiration .
	manualset3
164541	5	412325	7	NULL	NULL	0	NULL	ventilation/perfusion ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that fluctuations in the ethanol concentration are caused by variation in the ventilation/perfusion ratio of regions of the lung supplying the expirate , and that breath with ethanol in equilibrium with the plasma is not routinely obtained , especially at the end of a maximal expiration .
	manualset3
164542	6	412325	7	NULL	NULL	0	NULL	regions of the lung	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that fluctuations in the ethanol concentration are caused by variation in the ventilation/perfusion ratio of regions of the lung supplying the expirate , and that breath with ethanol in equilibrium with the plasma is not routinely obtained , especially at the end of a maximal expiration .
	manualset3
164543	7	412325	7	NULL	NULL	0	NULL	expirate	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that fluctuations in the ethanol concentration are caused by variation in the ventilation/perfusion ratio of regions of the lung supplying the expirate , and that breath with ethanol in equilibrium with the plasma is not routinely obtained , especially at the end of a maximal expiration .
	manualset3
164544	8	412325	7	NULL	NULL	0	NULL	breath	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that fluctuations in the ethanol concentration are caused by variation in the ventilation/perfusion ratio of regions of the lung supplying the expirate , and that breath with ethanol in equilibrium with the plasma is not routinely obtained , especially at the end of a maximal expiration .
	manualset3
164545	9	412325	7	NULL	NULL	0	NULL	ethanol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that fluctuations in the ethanol concentration are caused by variation in the ventilation/perfusion ratio of regions of the lung supplying the expirate , and that breath with ethanol in equilibrium with the plasma is not routinely obtained , especially at the end of a maximal expiration .
	manualset3
164546	10	412325	7	NULL	NULL	0	NULL	plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that fluctuations in the ethanol concentration are caused by variation in the ventilation/perfusion ratio of regions of the lung supplying the expirate , and that breath with ethanol in equilibrium with the plasma is not routinely obtained , especially at the end of a maximal expiration .
	manualset3
164547	11	412325	7	NULL	NULL	0	NULL	maximal expiration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that fluctuations in the ethanol concentration are caused by variation in the ventilation/perfusion ratio of regions of the lung supplying the expirate , and that breath with ethanol in equilibrium with the plasma is not routinely obtained , especially at the end of a maximal expiration .
	manualset3
164548	1	412326	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results suggest that inactivation of otherwise intact TP53 by aberrations in the proteasome pathway may contribute to the characteristic aneuploidy observed in OS .
	manualset3
164549	2	412326	7	NULL	NULL	0	NULL	inactivation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that inactivation of otherwise intact TP53 by aberrations in the proteasome pathway may contribute to the characteristic aneuploidy observed in OS .
	manualset3
164550	3	412326	7	NULL	NULL	NULL	NULL	intact TP53 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results suggest that inactivation of otherwise intact TP53 by aberrations in the proteasome pathway may contribute to the characteristic aneuploidy observed in OS .
	manualset3
164551	4	412326	7	NULL	NULL	0	NULL	proteasome pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that inactivation of otherwise intact TP53 by aberrations in the proteasome pathway may contribute to the characteristic aneuploidy observed in OS .
	manualset3
164552	5	412326	7	NULL	NULL	0	NULL	aneuploidy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that inactivation of otherwise intact TP53 by aberrations in the proteasome pathway may contribute to the characteristic aneuploidy observed in OS .
	manualset3
164553	6	412326	7	NULL	NULL	NULL	NULL	OS	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results suggest that inactivation of otherwise intact TP53 by aberrations in the proteasome pathway may contribute to the characteristic aneuploidy observed in OS .
	manualset3
164554	1	412327	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results suggest that resistance of B. cinerea to pyraclostrobin and boscalid was stable in the absence of the fungicides and that resistance to the two fungicides did not significantly impair individual fitness components tested .
	manualset3
164555	2	412327	7	NULL	NULL	0	NULL	resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that resistance of B. cinerea to pyraclostrobin and boscalid was stable in the absence of the fungicides and that resistance to the two fungicides did not significantly impair individual fitness components tested .
	manualset3
164556	3	412327	7	NULL	NULL	0	NULL	B. cinerea	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that resistance of B. cinerea to pyraclostrobin and boscalid was stable in the absence of the fungicides and that resistance to the two fungicides did not significantly impair individual fitness components tested .
	manualset3
164557	4	412327	7	NULL	NULL	0	NULL	pyraclostrobin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that resistance of B. cinerea to pyraclostrobin and boscalid was stable in the absence of the fungicides and that resistance to the two fungicides did not significantly impair individual fitness components tested .
	manualset3
164558	5	412327	7	NULL	NULL	0	NULL	boscalid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that resistance of B. cinerea to pyraclostrobin and boscalid was stable in the absence of the fungicides and that resistance to the two fungicides did not significantly impair individual fitness components tested .
	manualset3
164559	6	412327	7	NULL	NULL	NULL	NULL	absence 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results suggest that resistance of B. cinerea to pyraclostrobin and boscalid was stable in the absence of the fungicides and that resistance to the two fungicides did not significantly impair individual fitness components tested .
	manualset3
164560	7	412327	7	NULL	NULL	0	NULL	fungicides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that resistance of B. cinerea to pyraclostrobin and boscalid was stable in the absence of the fungicides and that resistance to the two fungicides did not significantly impair individual fitness components tested .
	manualset3
164561	8	412327	7	NULL	NULL	0	NULL	resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that resistance of B. cinerea to pyraclostrobin and boscalid was stable in the absence of the fungicides and that resistance to the two fungicides did not significantly impair individual fitness components tested .
	manualset3
164562	9	412327	7	NULL	NULL	0	NULL	two 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that resistance of B. cinerea to pyraclostrobin and boscalid was stable in the absence of the fungicides and that resistance to the two fungicides did not significantly impair individual fitness components tested .
	manualset3
164563	10	412327	7	NULL	NULL	0	NULL	fungicides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that resistance of B. cinerea to pyraclostrobin and boscalid was stable in the absence of the fungicides and that resistance to the two fungicides did not significantly impair individual fitness components tested .
	manualset3
164564	11	412327	7	NULL	NULL	NULL	NULL	individual fitness components	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results suggest that resistance of B. cinerea to pyraclostrobin and boscalid was stable in the absence of the fungicides and that resistance to the two fungicides did not significantly impair individual fitness components tested .
	manualset3
164565	1	412328	7	NULL	NULL	0	NULL	Clinico-electrophysiologic studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinico-electrophysiologic studies of the spastic syndrome and its neurosurgical treatment in patients with spinal cord lesions ) .
	manualset3
164566	2	412328	7	NULL	NULL	0	NULL	spastic syndrome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinico-electrophysiologic studies of the spastic syndrome and its neurosurgical treatment in patients with spinal cord lesions ) .
	manualset3
164567	3	412328	7	NULL	NULL	0	NULL	neurosurgical treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinico-electrophysiologic studies of the spastic syndrome and its neurosurgical treatment in patients with spinal cord lesions ) .
	manualset3
164568	4	412328	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinico-electrophysiologic studies of the spastic syndrome and its neurosurgical treatment in patients with spinal cord lesions ) .
	manualset3
164569	5	412328	7	NULL	NULL	0	NULL	 spinal cord lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinico-electrophysiologic studies of the spastic syndrome and its neurosurgical treatment in patients with spinal cord lesions ) .
	manualset3
164570	1	412329	7	NULL	NULL	0	NULL	Accidental and intentional perpetration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Accidental and intentional perpetration of serious injury or death : correlates and relationship to trauma exposure .
	manualset3
164571	2	412329	7	NULL	NULL	0	NULL	serious injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Accidental and intentional perpetration of serious injury or death : correlates and relationship to trauma exposure .
	manualset3
164572	3	412329	7	NULL	NULL	0	NULL	death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Accidental and intentional perpetration of serious injury or death : correlates and relationship to trauma exposure .
	manualset3
164573	4	412329	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Accidental and intentional perpetration of serious injury or death : correlates and relationship to trauma exposure .
	manualset3
164574	5	412329	7	NULL	NULL	0	NULL	 trauma exposure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Accidental and intentional perpetration of serious injury or death : correlates and relationship to trauma exposure .
	manualset3
164575	1	412330	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that swallowing sound is well characterized by a small number of dimensions .
	manualset3
164576	2	412330	7	NULL	NULL	0	NULL	swallowing sound	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that swallowing sound is well characterized by a small number of dimensions .
	manualset3
164577	3	412330	7	NULL	NULL	0	NULL	small number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that swallowing sound is well characterized by a small number of dimensions .
	manualset3
164578	4	412330	7	NULL	NULL	0	NULL	dimensions	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that swallowing sound is well characterized by a small number of dimensions .
	manualset3
164585	1	412331	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results suggest that the degree of enhanced tolerance to NaCl seems to require the induction of specific isoforms , depending on the different organelles .
	manualset3
164586	2	412331	7	NULL	NULL	0	NULL	degree	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that the degree of enhanced tolerance to NaCl seems to require the induction of specific isoforms , depending on the different organelles .
	manualset3
164587	3	412331	7	NULL	NULL	0	NULL	enhanced tolerance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that the degree of enhanced tolerance to NaCl seems to require the induction of specific isoforms , depending on the different organelles .
	manualset3
164588	4	412331	7	NULL	NULL	0	NULL	NaCl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that the degree of enhanced tolerance to NaCl seems to require the induction of specific isoforms , depending on the different organelles .
	manualset3
164589	5	412331	7	NULL	NULL	0	NULL	induction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that the degree of enhanced tolerance to NaCl seems to require the induction of specific isoforms , depending on the different organelles .
	manualset3
164590	6	412331	7	NULL	NULL	NULL	NULL	isoforms	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results suggest that the degree of enhanced tolerance to NaCl seems to require the induction of specific isoforms , depending on the different organelles .
	manualset3
164591	7	412331	7	NULL	NULL	0	NULL	organelles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that the degree of enhanced tolerance to NaCl seems to require the induction of specific isoforms , depending on the different organelles .
	manualset3
164592	1	412332	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results suggest that the effectiveness of sulfates in prolonging the antibacterial activity of teeth treated with chlorhexidine gluconate is related to the acidity and concentration of the sulfate solutions .
	manualset3
164593	2	412332	7	NULL	NULL	0	NULL	effectiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that the effectiveness of sulfates in prolonging the antibacterial activity of teeth treated with chlorhexidine gluconate is related to the acidity and concentration of the sulfate solutions .
	manualset3
164594	3	412332	7	NULL	NULL	0	NULL	sulfates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that the effectiveness of sulfates in prolonging the antibacterial activity of teeth treated with chlorhexidine gluconate is related to the acidity and concentration of the sulfate solutions .
	manualset3
164595	4	412332	7	NULL	NULL	0	NULL	antibacterial activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that the effectiveness of sulfates in prolonging the antibacterial activity of teeth treated with chlorhexidine gluconate is related to the acidity and concentration of the sulfate solutions .
	manualset3
164596	5	412332	7	NULL	NULL	0	NULL	 teeth	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that the effectiveness of sulfates in prolonging the antibacterial activity of teeth treated with chlorhexidine gluconate is related to the acidity and concentration of the sulfate solutions .
	manualset3
164597	6	412332	7	NULL	NULL	NULL	NULL	chlorhexidine gluconate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results suggest that the effectiveness of sulfates in prolonging the antibacterial activity of teeth treated with chlorhexidine gluconate is related to the acidity and concentration of the sulfate solutions .
	manualset3
164598	7	412332	7	NULL	NULL	0	NULL	acidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that the effectiveness of sulfates in prolonging the antibacterial activity of teeth treated with chlorhexidine gluconate is related to the acidity and concentration of the sulfate solutions .
	manualset3
164599	8	412332	7	NULL	NULL	0	NULL	concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that the effectiveness of sulfates in prolonging the antibacterial activity of teeth treated with chlorhexidine gluconate is related to the acidity and concentration of the sulfate solutions .
	manualset3
164600	9	412332	7	NULL	NULL	0	NULL	sulfate solutions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that the effectiveness of sulfates in prolonging the antibacterial activity of teeth treated with chlorhexidine gluconate is related to the acidity and concentration of the sulfate solutions .
	manualset3
164601	1	412333	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that the investigated doses of ICS 205-930 have only slight effects on gastric motor activity of healthy young men , with 20 mg reducing the rate of emptying .
	manualset3
164602	2	412333	7	NULL	NULL	0	NULL	doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that the investigated doses of ICS 205-930 have only slight effects on gastric motor activity of healthy young men , with 20 mg reducing the rate of emptying .
	manualset3
164603	3	412333	7	NULL	NULL	0	NULL	ICS 205-930	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that the investigated doses of ICS 205-930 have only slight effects on gastric motor activity of healthy young men , with 20 mg reducing the rate of emptying .
	manualset3
164604	4	412333	7	NULL	NULL	0	NULL	gastric motor activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that the investigated doses of ICS 205-930 have only slight effects on gastric motor activity of healthy young men , with 20 mg reducing the rate of emptying .
	manualset3
164605	5	412333	7	NULL	NULL	0	NULL	healthy young men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that the investigated doses of ICS 205-930 have only slight effects on gastric motor activity of healthy young men , with 20 mg reducing the rate of emptying .
	manualset3
164606	6	412333	7	NULL	NULL	0	NULL	20 mg	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that the investigated doses of ICS 205-930 have only slight effects on gastric motor activity of healthy young men , with 20 mg reducing the rate of emptying .
	manualset3
164607	7	412333	7	NULL	NULL	0	NULL	 rate of emptying	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that the investigated doses of ICS 205-930 have only slight effects on gastric motor activity of healthy young men , with 20 mg reducing the rate of emptying .
	manualset3
164608	1	412334	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that the resection of deposited material induces the improvement of the shoulder arthropathy .
	manualset3
164609	2	412334	7	NULL	NULL	0	NULL	resection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that the resection of deposited material induces the improvement of the shoulder arthropathy .
	manualset3
164610	3	412334	7	NULL	NULL	0	NULL	deposited material	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that the resection of deposited material induces the improvement of the shoulder arthropathy .
	manualset3
164611	4	412334	7	NULL	NULL	0	NULL	 improvement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that the resection of deposited material induces the improvement of the shoulder arthropathy .
	manualset3
164612	5	412334	7	NULL	NULL	0	NULL	shoulder arthropathy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that the resection of deposited material induces the improvement of the shoulder arthropathy .
	manualset3
164613	1	412335	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results suggest that there are specific CGRP receptors on afferent arterioles that produce relaxation and in glomeruli that are associated with an increase in cAMP production .
	manualset3
164614	2	412335	7	NULL	NULL	0	NULL	CGRP receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that there are specific CGRP receptors on afferent arterioles that produce relaxation and in glomeruli that are associated with an increase in cAMP production .
	manualset3
164615	3	412335	7	NULL	NULL	0	NULL	afferent arterioles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that there are specific CGRP receptors on afferent arterioles that produce relaxation and in glomeruli that are associated with an increase in cAMP production .
	manualset3
164616	4	412335	7	NULL	NULL	NULL	NULL	relaxation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results suggest that there are specific CGRP receptors on afferent arterioles that produce relaxation and in glomeruli that are associated with an increase in cAMP production .
	manualset3
164617	5	412335	7	NULL	NULL	0	NULL	glomeruli 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that there are specific CGRP receptors on afferent arterioles that produce relaxation and in glomeruli that are associated with an increase in cAMP production .
	manualset3
164618	6	412335	7	NULL	NULL	0	NULL	increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that there are specific CGRP receptors on afferent arterioles that produce relaxation and in glomeruli that are associated with an increase in cAMP production .
	manualset3
164619	7	412335	7	NULL	NULL	0	NULL	cAMP production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that there are specific CGRP receptors on afferent arterioles that produce relaxation and in glomeruli that are associated with an increase in cAMP production .
	manualset3
164620	1	412336	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results suggest that while community family planning clinics may provide effective services to the teenagers who seek them out , they may not be the most effective strategy for decreasing rates of pregnancy and childbearing in the overall teenage population .
	manualset3
164621	2	412336	7	NULL	NULL	0	NULL	community family planning clinics	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that while community family planning clinics may provide effective services to the teenagers who seek them out , they may not be the most effective strategy for decreasing rates of pregnancy and childbearing in the overall teenage population .
	manualset3
164622	3	412336	7	NULL	NULL	NULL	NULL	 services	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results suggest that while community family planning clinics may provide effective services to the teenagers who seek them out , they may not be the most effective strategy for decreasing rates of pregnancy and childbearing in the overall teenage population .
	manualset3
164623	4	412336	7	NULL	NULL	0	NULL	teenagers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that while community family planning clinics may provide effective services to the teenagers who seek them out , they may not be the most effective strategy for decreasing rates of pregnancy and childbearing in the overall teenage population .
	manualset3
164624	5	412336	7	NULL	NULL	0	NULL	strategy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that while community family planning clinics may provide effective services to the teenagers who seek them out , they may not be the most effective strategy for decreasing rates of pregnancy and childbearing in the overall teenage population .
	manualset3
164625	6	412336	7	NULL	NULL	0	NULL	decreasing rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that while community family planning clinics may provide effective services to the teenagers who seek them out , they may not be the most effective strategy for decreasing rates of pregnancy and childbearing in the overall teenage population .
	manualset3
164626	7	412336	7	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that while community family planning clinics may provide effective services to the teenagers who seek them out , they may not be the most effective strategy for decreasing rates of pregnancy and childbearing in the overall teenage population .
	manualset3
164627	8	412336	7	NULL	NULL	0	NULL	childbearing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that while community family planning clinics may provide effective services to the teenagers who seek them out , they may not be the most effective strategy for decreasing rates of pregnancy and childbearing in the overall teenage population .
	manualset3
164628	9	412336	7	NULL	NULL	0	NULL	teenage population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest that while community family planning clinics may provide effective services to the teenagers who seek them out , they may not be the most effective strategy for decreasing rates of pregnancy and childbearing in the overall teenage population .
	manualset3
164629	1	412337	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest the involvement of CC2D1A and CC2D2A in MR in the Han Chinese population , and some specific haplotypes may be susceptible or protective .
	manualset3
164630	2	412337	7	NULL	NULL	0	NULL	CC2D1A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest the involvement of CC2D1A and CC2D2A in MR in the Han Chinese population , and some specific haplotypes may be susceptible or protective .
	manualset3
164631	3	412337	7	NULL	NULL	0	NULL	CC2D2A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest the involvement of CC2D1A and CC2D2A in MR in the Han Chinese population , and some specific haplotypes may be susceptible or protective .
	manualset3
164632	4	412337	7	NULL	NULL	0	NULL	MR	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest the involvement of CC2D1A and CC2D2A in MR in the Han Chinese population , and some specific haplotypes may be susceptible or protective .
	manualset3
164633	5	412337	7	NULL	NULL	0	NULL	Han Chinese population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest the involvement of CC2D1A and CC2D2A in MR in the Han Chinese population , and some specific haplotypes may be susceptible or protective .
	manualset3
164634	6	412337	7	NULL	NULL	0	NULL	haplotypes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The results suggest the involvement of CC2D1A and CC2D2A in MR in the Han Chinese population , and some specific haplotypes may be susceptible or protective .
	manualset3
164635	1	412338	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results validate that the enzymatic removal of the intracellular superoxide at acupoints could generate acupuncture-like effects , and indicate a possibility of the new method as a simple substitute to acupuncture and an insight of superoxide modulation along meridians for acupuncture mechanism .
	manualset3
164636	2	412338	7	NULL	NULL	0	NULL	enzymatic removal 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results validate that the enzymatic removal of the intracellular superoxide at acupoints could generate acupuncture-like effects , and indicate a possibility of the new method as a simple substitute to acupuncture and an insight of superoxide modulation along meridians for acupuncture mechanism .
	manualset3
164637	3	412338	7	NULL	NULL	0	NULL	intracellular superoxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results validate that the enzymatic removal of the intracellular superoxide at acupoints could generate acupuncture-like effects , and indicate a possibility of the new method as a simple substitute to acupuncture and an insight of superoxide modulation along meridians for acupuncture mechanism .
	manualset3
164638	4	412338	7	NULL	NULL	0	NULL	acupoints	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results validate that the enzymatic removal of the intracellular superoxide at acupoints could generate acupuncture-like effects , and indicate a possibility of the new method as a simple substitute to acupuncture and an insight of superoxide modulation along meridians for acupuncture mechanism .
	manualset3
164639	5	412338	7	NULL	NULL	0	NULL	acupuncture-like effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results validate that the enzymatic removal of the intracellular superoxide at acupoints could generate acupuncture-like effects , and indicate a possibility of the new method as a simple substitute to acupuncture and an insight of superoxide modulation along meridians for acupuncture mechanism .
	manualset3
164640	6	412338	7	NULL	NULL	0	NULL	new method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The results validate that the enzymatic removal of the intracellular superoxide at acupoints could generate acupuncture-like effects , and indicate a possibility of the new method as a simple substitute to acupuncture and an insight of superoxide modulation along meridians for acupuncture mechanism .
	manualset3
164641	7	412338	7	NULL	NULL	0	NULL	acupuncture 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results validate that the enzymatic removal of the intracellular superoxide at acupoints could generate acupuncture-like effects , and indicate a possibility of the new method as a simple substitute to acupuncture and an insight of superoxide modulation along meridians for acupuncture mechanism .
	manualset3
164642	8	412338	7	NULL	NULL	0	NULL	superoxide modulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results validate that the enzymatic removal of the intracellular superoxide at acupoints could generate acupuncture-like effects , and indicate a possibility of the new method as a simple substitute to acupuncture and an insight of superoxide modulation along meridians for acupuncture mechanism .
	manualset3
164643	9	412338	7	NULL	NULL	0	NULL	meridians	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results validate that the enzymatic removal of the intracellular superoxide at acupoints could generate acupuncture-like effects , and indicate a possibility of the new method as a simple substitute to acupuncture and an insight of superoxide modulation along meridians for acupuncture mechanism .
	manualset3
164644	10	412338	7	NULL	NULL	0	NULL	acupuncture mechanism	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results validate that the enzymatic removal of the intracellular superoxide at acupoints could generate acupuncture-like effects , and indicate a possibility of the new method as a simple substitute to acupuncture and an insight of superoxide modulation along meridians for acupuncture mechanism .
	manualset3
165866	11	412338	7	NULL	NULL	0	NULL	simple substitute	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results validate that the enzymatic removal of the intracellular superoxide at acupoints could generate acupuncture-like effects , and indicate a possibility of the new method as a simple substitute to acupuncture and an insight of superoxide modulation along meridians for acupuncture mechanism .
	manualset3
166494	12	412338	7	NULL	NULL	NULL	NULL	possibility	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results validate that the enzymatic removal of the intracellular superoxide at acupoints could generate acupuncture-like effects , and indicate a possibility of the new method as a simple substitute to acupuncture and an insight of superoxide modulation along meridians for acupuncture mechanism .
	manualset3
164645	1	412339	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results were analyzed in strata , by age and BMI to avoid factors resulting in confusion , no relationship between salt intake , BP and rest of the variables studied being found in our community .
	manualset3
164646	2	412339	7	NULL	NULL	NULL	NULL	 age	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results were analyzed in strata , by age and BMI to avoid factors resulting in confusion , no relationship between salt intake , BP and rest of the variables studied being found in our community .
	manualset3
164647	3	412339	7	NULL	NULL	0	NULL	BMI 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results were analyzed in strata , by age and BMI to avoid factors resulting in confusion , no relationship between salt intake , BP and rest of the variables studied being found in our community .
	manualset3
164648	4	412339	7	NULL	NULL	0	NULL	confusion	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results were analyzed in strata , by age and BMI to avoid factors resulting in confusion , no relationship between salt intake , BP and rest of the variables studied being found in our community .
	manualset3
164649	5	412339	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The results were analyzed in strata , by age and BMI to avoid factors resulting in confusion , no relationship between salt intake , BP and rest of the variables studied being found in our community .
	manualset3
164650	6	412339	7	NULL	NULL	NULL	NULL	salt intake	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results were analyzed in strata , by age and BMI to avoid factors resulting in confusion , no relationship between salt intake , BP and rest of the variables studied being found in our community .
	manualset3
164651	7	412339	7	NULL	NULL	NULL	NULL	BP	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results were analyzed in strata , by age and BMI to avoid factors resulting in confusion , no relationship between salt intake , BP and rest of the variables studied being found in our community .
	manualset3
164652	8	412339	7	NULL	NULL	0	NULL	variables	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results were analyzed in strata , by age and BMI to avoid factors resulting in confusion , no relationship between salt intake , BP and rest of the variables studied being found in our community .
	manualset3
164653	9	412339	7	NULL	NULL	0	NULL	community	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results were analyzed in strata , by age and BMI to avoid factors resulting in confusion , no relationship between salt intake , BP and rest of the variables studied being found in our community .
	manualset3
165867	10	412339	7	NULL	NULL	0	NULL	factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results were analyzed in strata , by age and BMI to avoid factors resulting in confusion , no relationship between salt intake , BP and rest of the variables studied being found in our community .
	manualset3
164654	1	412340	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results were as follows : ( table : see text ) The balloon-expandable ( Palmaz-Schatz ) stent significantly further reduced , and in fact effectively abolished , the obstructive renal artery lesion in comparison to balloon angioplasty ( PTRA ) .
	manualset3
164655	2	412340	7	NULL	NULL	0	NULL	balloon-expandable ( Palmaz-Schatz ) stent	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The results were as follows : ( table : see text ) The balloon-expandable ( Palmaz-Schatz ) stent significantly further reduced , and in fact effectively abolished , the obstructive renal artery lesion in comparison to balloon angioplasty ( PTRA ) .
	manualset3
164656	3	412340	7	NULL	NULL	0	NULL	obstructive renal artery lesion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results were as follows : ( table : see text ) The balloon-expandable ( Palmaz-Schatz ) stent significantly further reduced , and in fact effectively abolished , the obstructive renal artery lesion in comparison to balloon angioplasty ( PTRA ) .
	manualset3
164657	4	412340	7	NULL	NULL	0	NULL	balloon angioplasty ( PTRA )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results were as follows : ( table : see text ) The balloon-expandable ( Palmaz-Schatz ) stent significantly further reduced , and in fact effectively abolished , the obstructive renal artery lesion in comparison to balloon angioplasty ( PTRA ) .
	manualset3
165868	5	412340	7	NULL	NULL	0	NULL	table : see text	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	The results were as follows : ( table : see text ) The balloon-expandable ( Palmaz-Schatz ) stent significantly further reduced , and in fact effectively abolished , the obstructive renal artery lesion in comparison to balloon angioplasty ( PTRA ) .
	manualset3
166495	6	412340	7	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The results were as follows : ( table : see text ) The balloon-expandable ( Palmaz-Schatz ) stent significantly further reduced , and in fact effectively abolished , the obstructive renal artery lesion in comparison to balloon angioplasty ( PTRA ) .
	manualset3
164658	1	412341	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results were compared with those obtained from animals suffered from chronic immobilization stress ( IMO ) .
	manualset3
164659	2	412341	7	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results were compared with those obtained from animals suffered from chronic immobilization stress ( IMO ) .
	manualset3
164660	3	412341	7	NULL	NULL	NULL	NULL	chronic immobilization stress ( IMO )	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results were compared with those obtained from animals suffered from chronic immobilization stress ( IMO ) .
	manualset3
164661	1	412342	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results were discussed in reference to targeting malleable family risk factors during early childhood associated with patterns of AB and mental health disorders during adolescence .
	manualset3
164662	2	412342	7	NULL	NULL	0	NULL	reference	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results were discussed in reference to targeting malleable family risk factors during early childhood associated with patterns of AB and mental health disorders during adolescence .
	manualset3
164663	3	412342	7	NULL	NULL	0	NULL	family risk factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results were discussed in reference to targeting malleable family risk factors during early childhood associated with patterns of AB and mental health disorders during adolescence .
	manualset3
164664	4	412342	7	NULL	NULL	0	NULL	early childhood	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The results were discussed in reference to targeting malleable family risk factors during early childhood associated with patterns of AB and mental health disorders during adolescence .
	manualset3
164665	5	412342	7	NULL	NULL	0	NULL	patterns of AB	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results were discussed in reference to targeting malleable family risk factors during early childhood associated with patterns of AB and mental health disorders during adolescence .
	manualset3
164666	6	412342	7	NULL	NULL	NULL	NULL	mental health disorders	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results were discussed in reference to targeting malleable family risk factors during early childhood associated with patterns of AB and mental health disorders during adolescence .
	manualset3
164667	7	412342	7	NULL	NULL	0	NULL	adolescence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results were discussed in reference to targeting malleable family risk factors during early childhood associated with patterns of AB and mental health disorders during adolescence .
	manualset3
164668	1	412343	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results were not attributable to a single bout of exercise since the gonadotrophin responses immediately or 24 h after such exercise did not parallel the results observed in the trained rats .
	manualset3
164669	2	412343	7	NULL	NULL	NULL	NULL	 single bout 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results were not attributable to a single bout of exercise since the gonadotrophin responses immediately or 24 h after such exercise did not parallel the results observed in the trained rats .
	manualset3
164670	4	412343	7	NULL	NULL	NULL	NULL	 gonadotrophin responses	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results were not attributable to a single bout of exercise since the gonadotrophin responses immediately or 24 h after such exercise did not parallel the results observed in the trained rats .
	manualset3
164671	5	412343	7	NULL	NULL	NULL	NULL	24 h after such exercise	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results were not attributable to a single bout of exercise since the gonadotrophin responses immediately or 24 h after such exercise did not parallel the results observed in the trained rats .
	manualset3
164672	3	412343	7	NULL	NULL	NULL	NULL	exercise	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results were not attributable to a single bout of exercise since the gonadotrophin responses immediately or 24 h after such exercise did not parallel the results observed in the trained rats .
	manualset3
164673	6	412343	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results were not attributable to a single bout of exercise since the gonadotrophin responses immediately or 24 h after such exercise did not parallel the results observed in the trained rats .
	manualset3
164674	7	412343	7	NULL	NULL	0	NULL	trained rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results were not attributable to a single bout of exercise since the gonadotrophin responses immediately or 24 h after such exercise did not parallel the results observed in the trained rats .
	manualset3
164675	1	412344	7	NULL	NULL	0	NULL	Accidents	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Accidents caused by a high-protein flour ) .
	manualset3
164676	2	412344	7	NULL	NULL	0	NULL	high-protein flour 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Accidents caused by a high-protein flour ) .
	manualset3
164677	1	412345	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results with ALA + FeCl3 suggested that stimulation of intracellular production of heme was also effective in blocking the increase in ALA synthase mRNA caused by AIA .
	manualset3
164678	2	412345	7	NULL	NULL	0	NULL	ALA + FeCl3 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results with ALA + FeCl3 suggested that stimulation of intracellular production of heme was also effective in blocking the increase in ALA synthase mRNA caused by AIA .
	manualset3
164679	3	412345	7	NULL	NULL	0	NULL	stimulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results with ALA + FeCl3 suggested that stimulation of intracellular production of heme was also effective in blocking the increase in ALA synthase mRNA caused by AIA .
	manualset3
164680	4	412345	7	NULL	NULL	0	NULL	intracellular production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results with ALA + FeCl3 suggested that stimulation of intracellular production of heme was also effective in blocking the increase in ALA synthase mRNA caused by AIA .
	manualset3
164681	5	412345	7	NULL	NULL	0	NULL	heme	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results with ALA + FeCl3 suggested that stimulation of intracellular production of heme was also effective in blocking the increase in ALA synthase mRNA caused by AIA .
	manualset3
164682	6	412345	7	NULL	NULL	0	NULL	 increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results with ALA + FeCl3 suggested that stimulation of intracellular production of heme was also effective in blocking the increase in ALA synthase mRNA caused by AIA .
	manualset3
164683	7	412345	7	NULL	NULL	0	NULL	ALA synthase mRNA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The results with ALA + FeCl3 suggested that stimulation of intracellular production of heme was also effective in blocking the increase in ALA synthase mRNA caused by AIA .
	manualset3
164684	8	412345	7	NULL	NULL	0	NULL	AIA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results with ALA + FeCl3 suggested that stimulation of intracellular production of heme was also effective in blocking the increase in ALA synthase mRNA caused by AIA .
	manualset3
164685	1	412346	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results would suggest that within this period of time a massive single bolus of ZON is nearly completely eliminated from the body .
	manualset3
164686	2	412346	7	NULL	NULL	NULL	NULL	 period of time	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results would suggest that within this period of time a massive single bolus of ZON is nearly completely eliminated from the body .
	manualset3
164687	3	412346	7	NULL	NULL	0	NULL	massive single bolus	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results would suggest that within this period of time a massive single bolus of ZON is nearly completely eliminated from the body .
	manualset3
164688	4	412346	7	NULL	NULL	0	NULL	ZON	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results would suggest that within this period of time a massive single bolus of ZON is nearly completely eliminated from the body .
	manualset3
164689	5	412346	7	NULL	NULL	0	NULL	body	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results would suggest that within this period of time a massive single bolus of ZON is nearly completely eliminated from the body .
	manualset3
164690	1	412347	7	NULL	NULL	0	NULL	reticulocyte cell membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The reticulocyte cell membrane was investigated for the role that it plays in cellular protein synthesis .
	manualset3
164691	2	412347	7	NULL	NULL	0	NULL	 role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The reticulocyte cell membrane was investigated for the role that it plays in cellular protein synthesis .
	manualset3
164692	3	412347	7	NULL	NULL	0	NULL	cellular protein synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The reticulocyte cell membrane was investigated for the role that it plays in cellular protein synthesis .
	manualset3
164693	1	412348	7	NULL	NULL	0	NULL	retinal distribution	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The retinal distribution of large ganglion cells appear to suggest certain similarities to mammalian alpha type ganglion cells .
	manualset3
164694	2	412348	7	NULL	NULL	0	NULL	large ganglion cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The retinal distribution of large ganglion cells appear to suggest certain similarities to mammalian alpha type ganglion cells .
	manualset3
164696	4	412348	7	NULL	NULL	NULL	NULL	mammalian alpha type ganglion cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The retinal distribution of large ganglion cells appear to suggest certain similarities to mammalian alpha type ganglion cells .
	manualset3
164697	3	412348	7	NULL	NULL	0	NULL	similarities	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The retinal distribution of large ganglion cells appear to suggest certain similarities to mammalian alpha type ganglion cells .
	manualset3
164698	1	412349	7	NULL	NULL	0	NULL	 retirement community 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The retirement community as a care alternative for the elderly .
	manualset3
164699	2	412349	7	NULL	NULL	0	NULL	care	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The retirement community as a care alternative for the elderly .
	manualset3
164700	3	412349	7	NULL	NULL	0	NULL	elderly	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The retirement community as a care alternative for the elderly .
	manualset3
164701	1	412350	7	NULL	NULL	0	NULL	retrograde tracer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The retrograde tracer FluoroGold was injected into the preoptic area of nine OVX ewes and labeled cells were examined in the brainstem to determine the extent of co-localization of ER .
	manualset3
164702	2	412350	7	NULL	NULL	0	NULL	FluoroGold 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The retrograde tracer FluoroGold was injected into the preoptic area of nine OVX ewes and labeled cells were examined in the brainstem to determine the extent of co-localization of ER .
	manualset3
164703	3	412350	7	NULL	NULL	0	NULL	preoptic area	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The retrograde tracer FluoroGold was injected into the preoptic area of nine OVX ewes and labeled cells were examined in the brainstem to determine the extent of co-localization of ER .
	manualset3
164704	4	412350	7	NULL	NULL	0	NULL	nine OVX ewes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The retrograde tracer FluoroGold was injected into the preoptic area of nine OVX ewes and labeled cells were examined in the brainstem to determine the extent of co-localization of ER .
	manualset3
164705	5	412350	7	NULL	NULL	0	NULL	labeled cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The retrograde tracer FluoroGold was injected into the preoptic area of nine OVX ewes and labeled cells were examined in the brainstem to determine the extent of co-localization of ER .
	manualset3
164706	6	412350	7	NULL	NULL	0	NULL	 brainstem	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The retrograde tracer FluoroGold was injected into the preoptic area of nine OVX ewes and labeled cells were examined in the brainstem to determine the extent of co-localization of ER .
	manualset3
164707	7	412350	7	NULL	NULL	NULL	NULL	extent	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The retrograde tracer FluoroGold was injected into the preoptic area of nine OVX ewes and labeled cells were examined in the brainstem to determine the extent of co-localization of ER .
	manualset3
164708	8	412350	7	NULL	NULL	0	NULL	co-localization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The retrograde tracer FluoroGold was injected into the preoptic area of nine OVX ewes and labeled cells were examined in the brainstem to determine the extent of co-localization of ER .
	manualset3
164709	9	412350	7	NULL	NULL	0	NULL	ER	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The retrograde tracer FluoroGold was injected into the preoptic area of nine OVX ewes and labeled cells were examined in the brainstem to determine the extent of co-localization of ER .
	manualset3
164710	1	412351	7	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The review also covers the recent progress achieved in the area of optical sensors based on MIPs .
	manualset3
164711	2	412351	7	NULL	NULL	0	NULL	progress	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The review also covers the recent progress achieved in the area of optical sensors based on MIPs .
	manualset3
164712	3	412351	7	NULL	NULL	NULL	NULL	area	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The review also covers the recent progress achieved in the area of optical sensors based on MIPs .
	manualset3
164713	4	412351	7	NULL	NULL	0	NULL	optical sensors	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The review also covers the recent progress achieved in the area of optical sensors based on MIPs .
	manualset3
164714	5	412351	7	NULL	NULL	0	NULL	MIPs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The review also covers the recent progress achieved in the area of optical sensors based on MIPs .
	manualset3
164715	1	412352	7	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The review briefly summarizes the results of spin-label studies of conformational transitions in monomeric globins ( myoglobin , leghemoglobin , erythrocruorin ) as well as in another heme-containing protein , cytochrome c , induced by heme ligands and pH. .
	manualset3
164716	2	412352	7	NULL	NULL	0	NULL	results	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The review briefly summarizes the results of spin-label studies of conformational transitions in monomeric globins ( myoglobin , leghemoglobin , erythrocruorin ) as well as in another heme-containing protein , cytochrome c , induced by heme ligands and pH. .
	manualset3
164717	3	412352	7	NULL	NULL	0	NULL	spin-label studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The review briefly summarizes the results of spin-label studies of conformational transitions in monomeric globins ( myoglobin , leghemoglobin , erythrocruorin ) as well as in another heme-containing protein , cytochrome c , induced by heme ligands and pH. .
	manualset3
164718	4	412352	7	NULL	NULL	0	NULL	conformational transitions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The review briefly summarizes the results of spin-label studies of conformational transitions in monomeric globins ( myoglobin , leghemoglobin , erythrocruorin ) as well as in another heme-containing protein , cytochrome c , induced by heme ligands and pH. .
	manualset3
164719	5	412352	7	NULL	NULL	0	NULL	monomeric globins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The review briefly summarizes the results of spin-label studies of conformational transitions in monomeric globins ( myoglobin , leghemoglobin , erythrocruorin ) as well as in another heme-containing protein , cytochrome c , induced by heme ligands and pH. .
	manualset3
164720	6	412352	7	NULL	NULL	0	NULL	myoglobin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The review briefly summarizes the results of spin-label studies of conformational transitions in monomeric globins ( myoglobin , leghemoglobin , erythrocruorin ) as well as in another heme-containing protein , cytochrome c , induced by heme ligands and pH. .
	manualset3
164721	7	412352	7	NULL	NULL	0	NULL	leghemoglobin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The review briefly summarizes the results of spin-label studies of conformational transitions in monomeric globins ( myoglobin , leghemoglobin , erythrocruorin ) as well as in another heme-containing protein , cytochrome c , induced by heme ligands and pH. .
	manualset3
164722	8	412352	7	NULL	NULL	0	NULL	erythrocruorin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The review briefly summarizes the results of spin-label studies of conformational transitions in monomeric globins ( myoglobin , leghemoglobin , erythrocruorin ) as well as in another heme-containing protein , cytochrome c , induced by heme ligands and pH. .
	manualset3
164723	9	412352	7	NULL	NULL	0	NULL	heme-containing protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The review briefly summarizes the results of spin-label studies of conformational transitions in monomeric globins ( myoglobin , leghemoglobin , erythrocruorin ) as well as in another heme-containing protein , cytochrome c , induced by heme ligands and pH. .
	manualset3
164724	10	412352	7	NULL	NULL	0	NULL	cytochrome c	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The review briefly summarizes the results of spin-label studies of conformational transitions in monomeric globins ( myoglobin , leghemoglobin , erythrocruorin ) as well as in another heme-containing protein , cytochrome c , induced by heme ligands and pH. .
	manualset3
164725	11	412352	7	NULL	NULL	0	NULL	 heme ligands 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The review briefly summarizes the results of spin-label studies of conformational transitions in monomeric globins ( myoglobin , leghemoglobin , erythrocruorin ) as well as in another heme-containing protein , cytochrome c , induced by heme ligands and pH. .
	manualset3
164726	12	412352	7	NULL	NULL	0	NULL	pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The review briefly summarizes the results of spin-label studies of conformational transitions in monomeric globins ( myoglobin , leghemoglobin , erythrocruorin ) as well as in another heme-containing protein , cytochrome c , induced by heme ligands and pH. .
	manualset3
164727	1	412353	7	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The review finds that non-specialized cancer nurses report a lack of education and training with regard to cancer care and cancer treatments , which acts as a barrier to providing quality nursing care .
	manualset3
164728	2	412353	7	NULL	NULL	0	NULL	non-specialized cancer nurses	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The review finds that non-specialized cancer nurses report a lack of education and training with regard to cancer care and cancer treatments , which acts as a barrier to providing quality nursing care .
	manualset3
164729	3	412353	7	NULL	NULL	0	NULL	education	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The review finds that non-specialized cancer nurses report a lack of education and training with regard to cancer care and cancer treatments , which acts as a barrier to providing quality nursing care .
	manualset3
164730	4	412353	7	NULL	NULL	0	NULL	training 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The review finds that non-specialized cancer nurses report a lack of education and training with regard to cancer care and cancer treatments , which acts as a barrier to providing quality nursing care .
	manualset3
164731	5	412353	7	NULL	NULL	0	NULL	cancer care	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The review finds that non-specialized cancer nurses report a lack of education and training with regard to cancer care and cancer treatments , which acts as a barrier to providing quality nursing care .
	manualset3
164732	6	412353	7	NULL	NULL	0	NULL	cancer treatments	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The review finds that non-specialized cancer nurses report a lack of education and training with regard to cancer care and cancer treatments , which acts as a barrier to providing quality nursing care .
	manualset3
164733	7	412353	7	NULL	NULL	NULL	NULL	barrier	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The review finds that non-specialized cancer nurses report a lack of education and training with regard to cancer care and cancer treatments , which acts as a barrier to providing quality nursing care .
	manualset3
164734	8	412353	7	NULL	NULL	0	NULL	quality nursing care	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The review finds that non-specialized cancer nurses report a lack of education and training with regard to cancer care and cancer treatments , which acts as a barrier to providing quality nursing care .
	manualset3
164735	1	412354	7	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The review presents a comprehensive survey of recent developments of high-performance capillary electromigration methods , zone electrophoresis , ITP , IEF , affinity electrophoresis , EKC and electrochromatography , and their application to analysis , preparation and physicochemical characterization of peptides .
	manualset3
164736	2	412354	7	NULL	NULL	0	NULL	comprehensive survey 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The review presents a comprehensive survey of recent developments of high-performance capillary electromigration methods , zone electrophoresis , ITP , IEF , affinity electrophoresis , EKC and electrochromatography , and their application to analysis , preparation and physicochemical characterization of peptides .
	manualset3
164737	3	412354	7	NULL	NULL	0	NULL	developments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The review presents a comprehensive survey of recent developments of high-performance capillary electromigration methods , zone electrophoresis , ITP , IEF , affinity electrophoresis , EKC and electrochromatography , and their application to analysis , preparation and physicochemical characterization of peptides .
	manualset3
164738	4	412354	7	NULL	NULL	0	NULL	high-performance capillary electromigration methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The review presents a comprehensive survey of recent developments of high-performance capillary electromigration methods , zone electrophoresis , ITP , IEF , affinity electrophoresis , EKC and electrochromatography , and their application to analysis , preparation and physicochemical characterization of peptides .
	manualset3
164739	5	412354	7	NULL	NULL	0	NULL	zone electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The review presents a comprehensive survey of recent developments of high-performance capillary electromigration methods , zone electrophoresis , ITP , IEF , affinity electrophoresis , EKC and electrochromatography , and their application to analysis , preparation and physicochemical characterization of peptides .
	manualset3
164740	6	412354	7	NULL	NULL	0	NULL	ITP	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The review presents a comprehensive survey of recent developments of high-performance capillary electromigration methods , zone electrophoresis , ITP , IEF , affinity electrophoresis , EKC and electrochromatography , and their application to analysis , preparation and physicochemical characterization of peptides .
	manualset3
164741	7	412354	7	NULL	NULL	0	NULL	IEF	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The review presents a comprehensive survey of recent developments of high-performance capillary electromigration methods , zone electrophoresis , ITP , IEF , affinity electrophoresis , EKC and electrochromatography , and their application to analysis , preparation and physicochemical characterization of peptides .
	manualset3
164742	8	412354	7	NULL	NULL	0	NULL	affinity electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The review presents a comprehensive survey of recent developments of high-performance capillary electromigration methods , zone electrophoresis , ITP , IEF , affinity electrophoresis , EKC and electrochromatography , and their application to analysis , preparation and physicochemical characterization of peptides .
	manualset3
164743	9	412354	7	NULL	NULL	0	NULL	EKC 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The review presents a comprehensive survey of recent developments of high-performance capillary electromigration methods , zone electrophoresis , ITP , IEF , affinity electrophoresis , EKC and electrochromatography , and their application to analysis , preparation and physicochemical characterization of peptides .
	manualset3
164744	10	412354	7	NULL	NULL	0	NULL	electrochromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The review presents a comprehensive survey of recent developments of high-performance capillary electromigration methods , zone electrophoresis , ITP , IEF , affinity electrophoresis , EKC and electrochromatography , and their application to analysis , preparation and physicochemical characterization of peptides .
	manualset3
164745	11	412354	7	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The review presents a comprehensive survey of recent developments of high-performance capillary electromigration methods , zone electrophoresis , ITP , IEF , affinity electrophoresis , EKC and electrochromatography , and their application to analysis , preparation and physicochemical characterization of peptides .
	manualset3
164746	12	412354	7	NULL	NULL	0	NULL	preparation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The review presents a comprehensive survey of recent developments of high-performance capillary electromigration methods , zone electrophoresis , ITP , IEF , affinity electrophoresis , EKC and electrochromatography , and their application to analysis , preparation and physicochemical characterization of peptides .
	manualset3
164747	13	412354	7	NULL	NULL	0	NULL	 physicochemical characterization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The review presents a comprehensive survey of recent developments of high-performance capillary electromigration methods , zone electrophoresis , ITP , IEF , affinity electrophoresis , EKC and electrochromatography , and their application to analysis , preparation and physicochemical characterization of peptides .
	manualset3
164748	14	412354	7	NULL	NULL	0	NULL	peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The review presents a comprehensive survey of recent developments of high-performance capillary electromigration methods , zone electrophoresis , ITP , IEF , affinity electrophoresis , EKC and electrochromatography , and their application to analysis , preparation and physicochemical characterization of peptides .
	manualset3
164749	1	412355	7	NULL	NULL	0	NULL	revised item stems	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The revised item stems were tested with a sample of 201 women , ages 35 to 95 .
	manualset3
164750	2	412355	7	NULL	NULL	0	NULL	sample	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The revised item stems were tested with a sample of 201 women , ages 35 to 95 .
	manualset3
164751	3	412355	7	NULL	NULL	0	NULL	201 women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The revised item stems were tested with a sample of 201 women , ages 35 to 95 .
	manualset3
164752	4	412355	7	NULL	NULL	0	NULL	ages 35 to 95	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The revised item stems were tested with a sample of 201 women , ages 35 to 95 .
	manualset3
164753	1	412356	7	NULL	NULL	0	NULL	 rhinoceros beetle	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The rhinoceros beetle , Oryctes rhinoceros , has emerged as a serious pest of oil palm since the prohibition of burning as a method for maintaining estate hygiene in the 1990s .
	manualset3
164754	2	412356	7	NULL	NULL	0	NULL	 Oryctes rhinoceros	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The rhinoceros beetle , Oryctes rhinoceros , has emerged as a serious pest of oil palm since the prohibition of burning as a method for maintaining estate hygiene in the 1990s .
	manualset3
164755	3	412356	7	NULL	NULL	0	NULL	serious pest	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The rhinoceros beetle , Oryctes rhinoceros , has emerged as a serious pest of oil palm since the prohibition of burning as a method for maintaining estate hygiene in the 1990s .
	manualset3
164756	4	412356	7	NULL	NULL	0	NULL	oil palm	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The rhinoceros beetle , Oryctes rhinoceros , has emerged as a serious pest of oil palm since the prohibition of burning as a method for maintaining estate hygiene in the 1990s .
	manualset3
164757	5	412356	7	NULL	NULL	0	NULL	prohibition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The rhinoceros beetle , Oryctes rhinoceros , has emerged as a serious pest of oil palm since the prohibition of burning as a method for maintaining estate hygiene in the 1990s .
	manualset3
164758	6	412356	7	NULL	NULL	0	NULL	burning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The rhinoceros beetle , Oryctes rhinoceros , has emerged as a serious pest of oil palm since the prohibition of burning as a method for maintaining estate hygiene in the 1990s .
	manualset3
164759	7	412356	7	NULL	NULL	0	NULL	method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The rhinoceros beetle , Oryctes rhinoceros , has emerged as a serious pest of oil palm since the prohibition of burning as a method for maintaining estate hygiene in the 1990s .
	manualset3
164760	8	412356	7	NULL	NULL	0	NULL	estate	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The rhinoceros beetle , Oryctes rhinoceros , has emerged as a serious pest of oil palm since the prohibition of burning as a method for maintaining estate hygiene in the 1990s .
	manualset3
164761	9	412356	7	NULL	NULL	NULL	NULL	hygiene	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The rhinoceros beetle , Oryctes rhinoceros , has emerged as a serious pest of oil palm since the prohibition of burning as a method for maintaining estate hygiene in the 1990s .
	manualset3
164762	10	412356	7	NULL	NULL	0	NULL	1990s	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The rhinoceros beetle , Oryctes rhinoceros , has emerged as a serious pest of oil palm since the prohibition of burning as a method for maintaining estate hygiene in the 1990s .
	manualset3
164763	1	412357	7	NULL	NULL	0	NULL	right graft	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The right graft retains the portal trunk , the common bile duct and the right branch of the hepatic artery .
	manualset3
164764	2	412357	7	NULL	NULL	0	NULL	portal trunk	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The right graft retains the portal trunk , the common bile duct and the right branch of the hepatic artery .
	manualset3
164765	3	412357	7	NULL	NULL	0	NULL	common bile duct 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The right graft retains the portal trunk , the common bile duct and the right branch of the hepatic artery .
	manualset3
164766	4	412357	7	NULL	NULL	0	NULL	right branch of the hepatic artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The right graft retains the portal trunk , the common bile duct and the right branch of the hepatic artery .
	manualset3
164767	1	412358	7	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of HIV infection from a blood transfusion is less than 1 in 100 , 000 in the United States .
	manualset3
164768	2	412358	7	NULL	NULL	0	NULL	HIV infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of HIV infection from a blood transfusion is less than 1 in 100 , 000 in the United States .
	manualset3
164769	3	412358	7	NULL	NULL	0	NULL	blood transfusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of HIV infection from a blood transfusion is less than 1 in 100 , 000 in the United States .
	manualset3
164770	4	412358	7	NULL	NULL	0	NULL	1 in 100 , 000	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of HIV infection from a blood transfusion is less than 1 in 100 , 000 in the United States .
	manualset3
164771	5	412358	7	NULL	NULL	0	NULL	United States	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of HIV infection from a blood transfusion is less than 1 in 100 , 000 in the United States .
	manualset3
164772	1	412359	7	NULL	NULL	0	NULL	risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of injury and death is increased by nearly six times ( OR = 5.58 , 95 % CI = 4.54-6 .85 ) for those who suffered a sudden illness while driving when compared to those non-sufferers .
	manualset3
164773	2	412359	7	NULL	NULL	0	NULL	injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of injury and death is increased by nearly six times ( OR = 5.58 , 95 % CI = 4.54-6 .85 ) for those who suffered a sudden illness while driving when compared to those non-sufferers .
	manualset3
164774	3	412359	7	NULL	NULL	0	NULL	death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of injury and death is increased by nearly six times ( OR = 5.58 , 95 % CI = 4.54-6 .85 ) for those who suffered a sudden illness while driving when compared to those non-sufferers .
	manualset3
164775	4	412359	7	NULL	NULL	0	NULL	six times	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of injury and death is increased by nearly six times ( OR = 5.58 , 95 % CI = 4.54-6 .85 ) for those who suffered a sudden illness while driving when compared to those non-sufferers .
	manualset3
164776	5	412359	7	NULL	NULL	0	NULL	OR = 5.58 , 95 % CI = 4.54-6 .85	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of injury and death is increased by nearly six times ( OR = 5.58 , 95 % CI = 4.54-6 .85 ) for those who suffered a sudden illness while driving when compared to those non-sufferers .
	manualset3
164777	6	412359	7	NULL	NULL	0	NULL	sudden illness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of injury and death is increased by nearly six times ( OR = 5.58 , 95 % CI = 4.54-6 .85 ) for those who suffered a sudden illness while driving when compared to those non-sufferers .
	manualset3
164778	7	412359	7	NULL	NULL	0	NULL	driving	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of injury and death is increased by nearly six times ( OR = 5.58 , 95 % CI = 4.54-6 .85 ) for those who suffered a sudden illness while driving when compared to those non-sufferers .
	manualset3
164779	8	412359	7	NULL	NULL	0	NULL	non-sufferers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of injury and death is increased by nearly six times ( OR = 5.58 , 95 % CI = 4.54-6 .85 ) for those who suffered a sudden illness while driving when compared to those non-sufferers .
	manualset3
164780	1	412360	7	NULL	NULL	0	NULL	risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of phenotypic abnormality from a de novo reciprocal translocation of inversion has been estimated at approximately 7 % ( Warburton , 1991 ) .
	manualset3
164781	2	412360	7	NULL	NULL	0	NULL	 phenotypic abnormality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of phenotypic abnormality from a de novo reciprocal translocation of inversion has been estimated at approximately 7 % ( Warburton , 1991 ) .
	manualset3
164782	3	412360	7	NULL	NULL	0	NULL	de novo reciprocal translocation of inversion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of phenotypic abnormality from a de novo reciprocal translocation of inversion has been estimated at approximately 7 % ( Warburton , 1991 ) .
	manualset3
164783	4	412360	7	NULL	NULL	0	NULL	 7 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of phenotypic abnormality from a de novo reciprocal translocation of inversion has been estimated at approximately 7 % ( Warburton , 1991 ) .
	manualset3
164784	5	412360	7	NULL	NULL	0	NULL	Warburton	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of phenotypic abnormality from a de novo reciprocal translocation of inversion has been estimated at approximately 7 % ( Warburton , 1991 ) .
	manualset3
164785	6	412360	7	NULL	NULL	0	NULL	1991	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of phenotypic abnormality from a de novo reciprocal translocation of inversion has been estimated at approximately 7 % ( Warburton , 1991 ) .
	manualset3
164786	1	412361	7	NULL	NULL	0	NULL	 risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of preeclampsia decreased across increasing quartiles of concentrations for retinol ( odds ratio of the highest quartile = 0.32 ; 95 % confidence interval : 0.15 , 0.69 , with the lowest quartile as the reference group ; p value of the test of linear trend = 0.001 ) .
	manualset3
164787	2	412361	7	NULL	NULL	0	NULL	preeclampsia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of preeclampsia decreased across increasing quartiles of concentrations for retinol ( odds ratio of the highest quartile = 0.32 ; 95 % confidence interval : 0.15 , 0.69 , with the lowest quartile as the reference group ; p value of the test of linear trend = 0.001 ) .
	manualset3
164788	3	412361	7	NULL	NULL	0	NULL	 increasing quartiles	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of preeclampsia decreased across increasing quartiles of concentrations for retinol ( odds ratio of the highest quartile = 0.32 ; 95 % confidence interval : 0.15 , 0.69 , with the lowest quartile as the reference group ; p value of the test of linear trend = 0.001 ) .
	manualset3
164789	4	412361	7	NULL	NULL	0	NULL	concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of preeclampsia decreased across increasing quartiles of concentrations for retinol ( odds ratio of the highest quartile = 0.32 ; 95 % confidence interval : 0.15 , 0.69 , with the lowest quartile as the reference group ; p value of the test of linear trend = 0.001 ) .
	manualset3
164790	5	412361	7	NULL	NULL	0	NULL	 retinol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of preeclampsia decreased across increasing quartiles of concentrations for retinol ( odds ratio of the highest quartile = 0.32 ; 95 % confidence interval : 0.15 , 0.69 , with the lowest quartile as the reference group ; p value of the test of linear trend = 0.001 ) .
	manualset3
164791	6	412361	7	NULL	NULL	0	NULL	odds ratio of the highest quartile	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of preeclampsia decreased across increasing quartiles of concentrations for retinol ( odds ratio of the highest quartile = 0.32 ; 95 % confidence interval : 0.15 , 0.69 , with the lowest quartile as the reference group ; p value of the test of linear trend = 0.001 ) .
	manualset3
164792	7	412361	7	NULL	NULL	0	NULL	0.32	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of preeclampsia decreased across increasing quartiles of concentrations for retinol ( odds ratio of the highest quartile = 0.32 ; 95 % confidence interval : 0.15 , 0.69 , with the lowest quartile as the reference group ; p value of the test of linear trend = 0.001 ) .
	manualset3
164793	8	412361	7	NULL	NULL	0	NULL	95 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of preeclampsia decreased across increasing quartiles of concentrations for retinol ( odds ratio of the highest quartile = 0.32 ; 95 % confidence interval : 0.15 , 0.69 , with the lowest quartile as the reference group ; p value of the test of linear trend = 0.001 ) .
	manualset3
164794	9	412361	7	NULL	NULL	0	NULL	confidence interval	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of preeclampsia decreased across increasing quartiles of concentrations for retinol ( odds ratio of the highest quartile = 0.32 ; 95 % confidence interval : 0.15 , 0.69 , with the lowest quartile as the reference group ; p value of the test of linear trend = 0.001 ) .
	manualset3
164795	10	412361	7	NULL	NULL	0	NULL	 0.15	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of preeclampsia decreased across increasing quartiles of concentrations for retinol ( odds ratio of the highest quartile = 0.32 ; 95 % confidence interval : 0.15 , 0.69 , with the lowest quartile as the reference group ; p value of the test of linear trend = 0.001 ) .
	manualset3
164796	11	412361	7	NULL	NULL	0	NULL	0.69	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of preeclampsia decreased across increasing quartiles of concentrations for retinol ( odds ratio of the highest quartile = 0.32 ; 95 % confidence interval : 0.15 , 0.69 , with the lowest quartile as the reference group ; p value of the test of linear trend = 0.001 ) .
	manualset3
164797	12	412361	7	NULL	NULL	0	NULL	lowest quartile	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of preeclampsia decreased across increasing quartiles of concentrations for retinol ( odds ratio of the highest quartile = 0.32 ; 95 % confidence interval : 0.15 , 0.69 , with the lowest quartile as the reference group ; p value of the test of linear trend = 0.001 ) .
	manualset3
164798	13	412361	7	NULL	NULL	NULL	NULL	reference group	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The risk of preeclampsia decreased across increasing quartiles of concentrations for retinol ( odds ratio of the highest quartile = 0.32 ; 95 % confidence interval : 0.15 , 0.69 , with the lowest quartile as the reference group ; p value of the test of linear trend = 0.001 ) .
	manualset3
164799	14	412361	7	NULL	NULL	NULL	NULL	 p value  	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The risk of preeclampsia decreased across increasing quartiles of concentrations for retinol ( odds ratio of the highest quartile = 0.32 ; 95 % confidence interval : 0.15 , 0.69 , with the lowest quartile as the reference group ; p value of the test of linear trend = 0.001 ) .
	manualset3
164800	16	412361	7	NULL	NULL	NULL	NULL	0.001	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The risk of preeclampsia decreased across increasing quartiles of concentrations for retinol ( odds ratio of the highest quartile = 0.32 ; 95 % confidence interval : 0.15 , 0.69 , with the lowest quartile as the reference group ; p value of the test of linear trend = 0.001 ) .
	manualset3
165870	15	412361	7	NULL	NULL	0	NULL	test of linear trend	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of preeclampsia decreased across increasing quartiles of concentrations for retinol ( odds ratio of the highest quartile = 0.32 ; 95 % confidence interval : 0.15 , 0.69 , with the lowest quartile as the reference group ; p value of the test of linear trend = 0.001 ) .
	manualset3
164801	1	412362	7	NULL	NULL	0	NULL	risks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The risks and benefits of the thiazide therapy should be considered before starting long-term treatment of children with hypercalciuria and haematuria or renal stone disease .
	manualset3
164802	2	412362	7	NULL	NULL	0	NULL	benefits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The risks and benefits of the thiazide therapy should be considered before starting long-term treatment of children with hypercalciuria and haematuria or renal stone disease .
	manualset3
164803	3	412362	7	NULL	NULL	0	NULL	thiazide therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The risks and benefits of the thiazide therapy should be considered before starting long-term treatment of children with hypercalciuria and haematuria or renal stone disease .
	manualset3
164804	4	412362	7	NULL	NULL	0	NULL	long-term treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The risks and benefits of the thiazide therapy should be considered before starting long-term treatment of children with hypercalciuria and haematuria or renal stone disease .
	manualset3
164805	5	412362	7	NULL	NULL	NULL	NULL	children	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The risks and benefits of the thiazide therapy should be considered before starting long-term treatment of children with hypercalciuria and haematuria or renal stone disease .
	manualset3
164806	6	412362	7	NULL	NULL	0	NULL	hypercalciuria 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The risks and benefits of the thiazide therapy should be considered before starting long-term treatment of children with hypercalciuria and haematuria or renal stone disease .
	manualset3
164807	7	412362	7	NULL	NULL	0	NULL	haematuria	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The risks and benefits of the thiazide therapy should be considered before starting long-term treatment of children with hypercalciuria and haematuria or renal stone disease .
	manualset3
164808	8	412362	7	NULL	NULL	0	NULL	renal stone disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The risks and benefits of the thiazide therapy should be considered before starting long-term treatment of children with hypercalciuria and haematuria or renal stone disease .
	manualset3
164809	1	412363	7	NULL	NULL	NULL	NULL	roentgenological diagnosis	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The roentgenological diagnosis corresponded morphologically with a proliferation of sub-mucous esophagus glands and a dilatation of their outlets , a portion of which displayed platelet epithelial metaplasia .
	manualset3
164810	2	412363	7	NULL	NULL	0	NULL	 proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The roentgenological diagnosis corresponded morphologically with a proliferation of sub-mucous esophagus glands and a dilatation of their outlets , a portion of which displayed platelet epithelial metaplasia .
	manualset3
164811	3	412363	7	NULL	NULL	0	NULL	sub-mucous esophagus glands	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The roentgenological diagnosis corresponded morphologically with a proliferation of sub-mucous esophagus glands and a dilatation of their outlets , a portion of which displayed platelet epithelial metaplasia .
	manualset3
164812	4	412363	7	NULL	NULL	0	NULL	dilatation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The roentgenological diagnosis corresponded morphologically with a proliferation of sub-mucous esophagus glands and a dilatation of their outlets , a portion of which displayed platelet epithelial metaplasia .
	manualset3
164813	5	412363	7	NULL	NULL	0	NULL	outlets	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The roentgenological diagnosis corresponded morphologically with a proliferation of sub-mucous esophagus glands and a dilatation of their outlets , a portion of which displayed platelet epithelial metaplasia .
	manualset3
164814	6	412363	7	NULL	NULL	0	NULL	portion	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The roentgenological diagnosis corresponded morphologically with a proliferation of sub-mucous esophagus glands and a dilatation of their outlets , a portion of which displayed platelet epithelial metaplasia .
	manualset3
164815	7	412363	7	NULL	NULL	0	NULL	platelet epithelial metaplasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The roentgenological diagnosis corresponded morphologically with a proliferation of sub-mucous esophagus glands and a dilatation of their outlets , a portion of which displayed platelet epithelial metaplasia .
	manualset3
164816	1	412364	7	NULL	NULL	NULL	NULL	 role	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The role of Apaf-1 in programmed cell death : from worm to tumor .
	manualset3
164817	2	412364	7	NULL	NULL	0	NULL	Apaf-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of Apaf-1 in programmed cell death : from worm to tumor .
	manualset3
164818	3	412364	7	NULL	NULL	0	NULL	programmed cell death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of Apaf-1 in programmed cell death : from worm to tumor .
	manualset3
164819	4	412364	7	NULL	NULL	0	NULL	worm 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of Apaf-1 in programmed cell death : from worm to tumor .
	manualset3
164820	5	412364	7	NULL	NULL	0	NULL	tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of Apaf-1 in programmed cell death : from worm to tumor .
	manualset3
164821	1	412365	7	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of CD40/CD154 interaction during infection has primarily focused on pathogens that drive inflammatory Th1 responses .
	manualset3
164822	2	412365	7	NULL	NULL	0	NULL	CD40/CD154 interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of CD40/CD154 interaction during infection has primarily focused on pathogens that drive inflammatory Th1 responses .
	manualset3
164823	3	412365	7	NULL	NULL	0	NULL	infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of CD40/CD154 interaction during infection has primarily focused on pathogens that drive inflammatory Th1 responses .
	manualset3
164824	4	412365	7	NULL	NULL	0	NULL	pathogens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of CD40/CD154 interaction during infection has primarily focused on pathogens that drive inflammatory Th1 responses .
	manualset3
164825	5	412365	7	NULL	NULL	0	NULL	inflammatory Th1 responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of CD40/CD154 interaction during infection has primarily focused on pathogens that drive inflammatory Th1 responses .
	manualset3
164826	1	412366	7	NULL	NULL	NULL	NULL	 role	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The role of CD44 in the acute and resolution phase of the host response during pneumococcal pneumonia .
	manualset3
164827	2	412366	7	NULL	NULL	0	NULL	CD44	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of CD44 in the acute and resolution phase of the host response during pneumococcal pneumonia .
	manualset3
164828	3	412366	7	NULL	NULL	0	NULL	acute phase	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of CD44 in the acute and resolution phase of the host response during pneumococcal pneumonia .
	manualset3
164829	4	412366	7	NULL	NULL	0	NULL	 resolution phase	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of CD44 in the acute and resolution phase of the host response during pneumococcal pneumonia .
	manualset3
164830	5	412366	7	NULL	NULL	0	NULL	host response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of CD44 in the acute and resolution phase of the host response during pneumococcal pneumonia .
	manualset3
164831	6	412366	7	NULL	NULL	0	NULL	pneumococcal pneumonia	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of CD44 in the acute and resolution phase of the host response during pneumococcal pneumonia .
	manualset3
164832	1	412367	7	NULL	NULL	0	NULL	role 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of Epstein-Barr virus ( EBV ) in the pathogenesis of severe , chronic active EBV infection and its complications is unclear .
	manualset3
164833	2	412367	7	NULL	NULL	0	NULL	Epstein-Barr virus ( EBV ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of Epstein-Barr virus ( EBV ) in the pathogenesis of severe , chronic active EBV infection and its complications is unclear .
	manualset3
164834	3	412367	7	NULL	NULL	0	NULL	pathogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of Epstein-Barr virus ( EBV ) in the pathogenesis of severe , chronic active EBV infection and its complications is unclear .
	manualset3
164835	4	412367	7	NULL	NULL	0	NULL	 severe , chronic active EBV infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of Epstein-Barr virus ( EBV ) in the pathogenesis of severe , chronic active EBV infection and its complications is unclear .
	manualset3
164836	5	412367	7	NULL	NULL	0	NULL	complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of Epstein-Barr virus ( EBV ) in the pathogenesis of severe , chronic active EBV infection and its complications is unclear .
	manualset3
164837	1	412368	7	NULL	NULL	0	NULL	 role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of Helicobacter pylori in the spectrum of Barrett 's carcinogenesis .
	manualset3
164838	2	412368	7	NULL	NULL	0	NULL	Helicobacter pylori 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of Helicobacter pylori in the spectrum of Barrett 's carcinogenesis .
	manualset3
164839	3	412368	7	NULL	NULL	0	NULL	spectrum	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of Helicobacter pylori in the spectrum of Barrett 's carcinogenesis .
	manualset3
164840	4	412368	7	NULL	NULL	0	NULL	Barrett 's carcinogenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of Helicobacter pylori in the spectrum of Barrett 's carcinogenesis .
	manualset3
164841	1	412369	7	NULL	NULL	0	NULL	role 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of SPINK1 mutations in modifying the expression of PRSS1mutations is unclear but appears to be of clinical importance .
	manualset3
164842	2	412369	7	NULL	NULL	0	NULL	SPINK1 mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of SPINK1 mutations in modifying the expression of PRSS1mutations is unclear but appears to be of clinical importance .
	manualset3
164843	3	412369	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of SPINK1 mutations in modifying the expression of PRSS1mutations is unclear but appears to be of clinical importance .
	manualset3
164844	4	412369	7	NULL	NULL	0	NULL	PRSS1mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of SPINK1 mutations in modifying the expression of PRSS1mutations is unclear but appears to be of clinical importance .
	manualset3
172016	5	412369	7	NULL	NULL	0	NULL	 clinical importance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of SPINK1 mutations in modifying the expression of PRSS1mutations is unclear but appears to be of clinical importance .
	manualset3
164845	1	412370	7	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of Xenopus Rx-L in photoreceptor cell determination .
	manualset3
164846	2	412370	7	NULL	NULL	NULL	NULL	Xenopus Rx-L	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The role of Xenopus Rx-L in photoreceptor cell determination .
	manualset3
164847	3	412370	7	NULL	NULL	0	NULL	photoreceptor cell determination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of Xenopus Rx-L in photoreceptor cell determination .
	manualset3
164848	1	412371	7	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of academic health centers in addressing social responsibility .
	manualset3
164849	2	412371	7	NULL	NULL	0	NULL	academic health centers	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of academic health centers in addressing social responsibility .
	manualset3
164850	3	412371	7	NULL	NULL	NULL	NULL	social responsibility	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The role of academic health centers in addressing social responsibility .
	manualset3
164851	1	412372	7	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of allergy and nonspecific airway hyperresponsiveness in the pathogenesis of chronic obstructive pulmonary disease .
	manualset3
164852	2	412372	7	NULL	NULL	0	NULL	allergy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of allergy and nonspecific airway hyperresponsiveness in the pathogenesis of chronic obstructive pulmonary disease .
	manualset3
164853	3	412372	7	NULL	NULL	0	NULL	 nonspecific airway hyperresponsiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of allergy and nonspecific airway hyperresponsiveness in the pathogenesis of chronic obstructive pulmonary disease .
	manualset3
164854	4	412372	7	NULL	NULL	0	NULL	pathogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of allergy and nonspecific airway hyperresponsiveness in the pathogenesis of chronic obstructive pulmonary disease .
	manualset3
164855	5	412372	7	NULL	NULL	0	NULL	chronic obstructive pulmonary disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of allergy and nonspecific airway hyperresponsiveness in the pathogenesis of chronic obstructive pulmonary disease .
	manualset3
164857	1	412373	7	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of altered `` vitamin D nutrition '' in leading to the observed greater incidence of secondary hyperparathyroidism in African Americans with ESRD compared to other racial groups is considered .
	manualset3
164858	2	412373	7	NULL	NULL	0	NULL	altered `` vitamin D nutrition ''	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of altered `` vitamin D nutrition '' in leading to the observed greater incidence of secondary hyperparathyroidism in African Americans with ESRD compared to other racial groups is considered .
	manualset3
164859	3	412373	7	NULL	NULL	0	NULL	 greater incidence 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of altered `` vitamin D nutrition '' in leading to the observed greater incidence of secondary hyperparathyroidism in African Americans with ESRD compared to other racial groups is considered .
	manualset3
164860	4	412373	7	NULL	NULL	0	NULL	secondary hyperparathyroidism	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of altered `` vitamin D nutrition '' in leading to the observed greater incidence of secondary hyperparathyroidism in African Americans with ESRD compared to other racial groups is considered .
	manualset3
164861	5	412373	7	NULL	NULL	0	NULL	 African Americans	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of altered `` vitamin D nutrition '' in leading to the observed greater incidence of secondary hyperparathyroidism in African Americans with ESRD compared to other racial groups is considered .
	manualset3
164862	6	412373	7	NULL	NULL	0	NULL	ESRD	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of altered `` vitamin D nutrition '' in leading to the observed greater incidence of secondary hyperparathyroidism in African Americans with ESRD compared to other racial groups is considered .
	manualset3
164863	7	412373	7	NULL	NULL	0	NULL	racial groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of altered `` vitamin D nutrition '' in leading to the observed greater incidence of secondary hyperparathyroidism in African Americans with ESRD compared to other racial groups is considered .
	manualset3
164864	1	412374	7	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of avastin in the management of recurrent glioblastoma .
	manualset3
164865	2	412374	7	NULL	NULL	0	NULL	 avastin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of avastin in the management of recurrent glioblastoma .
	manualset3
164866	3	412374	7	NULL	NULL	0	NULL	management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of avastin in the management of recurrent glioblastoma .
	manualset3
164867	4	412374	7	NULL	NULL	NULL	NULL	 recurrent glioblastoma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The role of avastin in the management of recurrent glioblastoma .
	manualset3
164868	1	412375	7	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of circadian proteins in regulating whole-body metabolism and bone turnover has been studied in detail and has led to the discovery of an elemental system for timekeeping involving the core genes Clock , Bmal1 , Per , and Cry .
	manualset3
164869	2	412375	7	NULL	NULL	0	NULL	circadian proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of circadian proteins in regulating whole-body metabolism and bone turnover has been studied in detail and has led to the discovery of an elemental system for timekeeping involving the core genes Clock , Bmal1 , Per , and Cry .
	manualset3
164870	3	412375	7	NULL	NULL	0	NULL	whole-body metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of circadian proteins in regulating whole-body metabolism and bone turnover has been studied in detail and has led to the discovery of an elemental system for timekeeping involving the core genes Clock , Bmal1 , Per , and Cry .
	manualset3
164871	4	412375	7	NULL	NULL	0	NULL	bone turnover	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of circadian proteins in regulating whole-body metabolism and bone turnover has been studied in detail and has led to the discovery of an elemental system for timekeeping involving the core genes Clock , Bmal1 , Per , and Cry .
	manualset3
164872	5	412375	7	NULL	NULL	0	NULL	discovery	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of circadian proteins in regulating whole-body metabolism and bone turnover has been studied in detail and has led to the discovery of an elemental system for timekeeping involving the core genes Clock , Bmal1 , Per , and Cry .
	manualset3
164873	6	412375	7	NULL	NULL	0	NULL	elemental system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of circadian proteins in regulating whole-body metabolism and bone turnover has been studied in detail and has led to the discovery of an elemental system for timekeeping involving the core genes Clock , Bmal1 , Per , and Cry .
	manualset3
164874	7	412375	7	NULL	NULL	0	NULL	timekeeping	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of circadian proteins in regulating whole-body metabolism and bone turnover has been studied in detail and has led to the discovery of an elemental system for timekeeping involving the core genes Clock , Bmal1 , Per , and Cry .
	manualset3
164875	8	412375	7	NULL	NULL	0	NULL	 core genes Clock	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of circadian proteins in regulating whole-body metabolism and bone turnover has been studied in detail and has led to the discovery of an elemental system for timekeeping involving the core genes Clock , Bmal1 , Per , and Cry .
	manualset3
164876	9	412375	7	NULL	NULL	0	NULL	core genes Bmal1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of circadian proteins in regulating whole-body metabolism and bone turnover has been studied in detail and has led to the discovery of an elemental system for timekeeping involving the core genes Clock , Bmal1 , Per , and Cry .
	manualset3
164877	10	412375	7	NULL	NULL	0	NULL	core genes Per	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of circadian proteins in regulating whole-body metabolism and bone turnover has been studied in detail and has led to the discovery of an elemental system for timekeeping involving the core genes Clock , Bmal1 , Per , and Cry .
	manualset3
164878	11	412375	7	NULL	NULL	0	NULL	core genes Cry	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of circadian proteins in regulating whole-body metabolism and bone turnover has been studied in detail and has led to the discovery of an elemental system for timekeeping involving the core genes Clock , Bmal1 , Per , and Cry .
	manualset3
164880	1	412376	7	NULL	NULL	0	NULL	role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of cisternal shunting in neurosurgical practice is discussed .
	manualset3
164881	2	412376	7	NULL	NULL	0	NULL	cisternal shunting	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of cisternal shunting in neurosurgical practice is discussed .
	manualset3
164882	3	412376	7	NULL	NULL	0	NULL	neurosurgical practice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of cisternal shunting in neurosurgical practice is discussed .
	manualset3
164883	1	412377	7	NULL	NULL	0	NULL	role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of endometrial contractility in displacing human embryos from the Fallopian tube to the lumen cavity of the uterus or vagina in terms of pregnancy or wastage is still a matter of discussion .
	manualset3
164884	2	412377	7	NULL	NULL	0	NULL	endometrial contractility	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of endometrial contractility in displacing human embryos from the Fallopian tube to the lumen cavity of the uterus or vagina in terms of pregnancy or wastage is still a matter of discussion .
	manualset3
164885	3	412377	7	NULL	NULL	0	NULL	human embryos	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of endometrial contractility in displacing human embryos from the Fallopian tube to the lumen cavity of the uterus or vagina in terms of pregnancy or wastage is still a matter of discussion .
	manualset3
164886	4	412377	7	NULL	NULL	0	NULL	Fallopian tube	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of endometrial contractility in displacing human embryos from the Fallopian tube to the lumen cavity of the uterus or vagina in terms of pregnancy or wastage is still a matter of discussion .
	manualset3
164887	5	412377	7	NULL	NULL	0	NULL	lumen cavity	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of endometrial contractility in displacing human embryos from the Fallopian tube to the lumen cavity of the uterus or vagina in terms of pregnancy or wastage is still a matter of discussion .
	manualset3
164888	6	412377	7	NULL	NULL	0	NULL	uterus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of endometrial contractility in displacing human embryos from the Fallopian tube to the lumen cavity of the uterus or vagina in terms of pregnancy or wastage is still a matter of discussion .
	manualset3
164889	7	412377	7	NULL	NULL	0	NULL	vagina	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of endometrial contractility in displacing human embryos from the Fallopian tube to the lumen cavity of the uterus or vagina in terms of pregnancy or wastage is still a matter of discussion .
	manualset3
164890	8	412377	7	NULL	NULL	0	NULL	pregnancy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of endometrial contractility in displacing human embryos from the Fallopian tube to the lumen cavity of the uterus or vagina in terms of pregnancy or wastage is still a matter of discussion .
	manualset3
164891	9	412377	7	NULL	NULL	0	NULL	wastage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of endometrial contractility in displacing human embryos from the Fallopian tube to the lumen cavity of the uterus or vagina in terms of pregnancy or wastage is still a matter of discussion .
	manualset3
164892	10	412377	7	NULL	NULL	0	NULL	discussion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of endometrial contractility in displacing human embryos from the Fallopian tube to the lumen cavity of the uterus or vagina in terms of pregnancy or wastage is still a matter of discussion .
	manualset3
164893	1	412378	7	NULL	NULL	0	NULL	role 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of estradiol in the maintenance of secondary hypogonadism in males in erectile dysfunction .
	manualset3
164894	2	412378	7	NULL	NULL	0	NULL	estradiol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of estradiol in the maintenance of secondary hypogonadism in males in erectile dysfunction .
	manualset3
164895	3	412378	7	NULL	NULL	0	NULL	secondary hypogonadism 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of estradiol in the maintenance of secondary hypogonadism in males in erectile dysfunction .
	manualset3
164896	4	412378	7	NULL	NULL	0	NULL	males 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of estradiol in the maintenance of secondary hypogonadism in males in erectile dysfunction .
	manualset3
164897	5	412378	7	NULL	NULL	0	NULL	erectile dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of estradiol in the maintenance of secondary hypogonadism in males in erectile dysfunction .
	manualset3
172017	6	412378	7	NULL	NULL	0	NULL	maintenance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of estradiol in the maintenance of secondary hypogonadism in males in erectile dysfunction .
	manualset3
164898	1	412379	7	NULL	NULL	0	NULL	role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of factor VII in the hemostatic mechanism as well as thrombosis has recently gained new interest .
	manualset3
164899	2	412379	7	NULL	NULL	0	NULL	factor VII	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of factor VII in the hemostatic mechanism as well as thrombosis has recently gained new interest .
	manualset3
164900	3	412379	7	NULL	NULL	0	NULL	hemostatic mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of factor VII in the hemostatic mechanism as well as thrombosis has recently gained new interest .
	manualset3
164901	4	412379	7	NULL	NULL	0	NULL	 thrombosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of factor VII in the hemostatic mechanism as well as thrombosis has recently gained new interest .
	manualset3
172018	5	412379	7	NULL	NULL	0	NULL	 interest	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of factor VII in the hemostatic mechanism as well as thrombosis has recently gained new interest .
	manualset3
164902	1	412380	7	NULL	NULL	0	NULL	role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of fetal hemoglobin-enhancing agents in thalassemia .
	manualset3
164903	2	412380	7	NULL	NULL	0	NULL	fetal hemoglobin-enhancing agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of fetal hemoglobin-enhancing agents in thalassemia .
	manualset3
164904	3	412380	7	NULL	NULL	0	NULL	thalassemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of fetal hemoglobin-enhancing agents in thalassemia .
	manualset3
164905	1	412381	7	NULL	NULL	NULL	NULL	 fimbriae 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The role of fimbriae in gaining entry into human DCs and how this modulates the inflammatory and effector immune responses , however , have not been explored .
	manualset3
164906	2	412381	7	NULL	NULL	0	NULL	human DCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of fimbriae in gaining entry into human DCs and how this modulates the inflammatory and effector immune responses , however , have not been explored .
	manualset3
164907	3	412381	7	NULL	NULL	0	NULL	 inflammatory immune response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of fimbriae in gaining entry into human DCs and how this modulates the inflammatory and effector immune responses , however , have not been explored .
	manualset3
164908	4	412381	7	NULL	NULL	0	NULL	effector immune responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of fimbriae in gaining entry into human DCs and how this modulates the inflammatory and effector immune responses , however , have not been explored .
	manualset3
165006	5	412381	7	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of fimbriae in gaining entry into human DCs and how this modulates the inflammatory and effector immune responses , however , have not been explored .
	manualset3
164909	1	412382	7	NULL	NULL	NULL	NULL	role	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The role of glyco ( geno ) lytic ATP production at high contraction workloads is discussed in the context of this result .
	manualset3
164910	2	412382	7	NULL	NULL	0	NULL	glyco ( geno ) lytic ATP production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of glyco ( geno ) lytic ATP production at high contraction workloads is discussed in the context of this result .
	manualset3
164911	3	412382	7	NULL	NULL	0	NULL	high contraction workloads	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of glyco ( geno ) lytic ATP production at high contraction workloads is discussed in the context of this result .
	manualset3
164912	4	412382	7	NULL	NULL	0	NULL	context	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of glyco ( geno ) lytic ATP production at high contraction workloads is discussed in the context of this result .
	manualset3
164913	5	412382	7	NULL	NULL	0	NULL	result	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of glyco ( geno ) lytic ATP production at high contraction workloads is discussed in the context of this result .
	manualset3
164914	1	412383	7	NULL	NULL	0	NULL	role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of history , Epworth Sleepiness Scale Score and body mass index in identifying non-apnoeic snorers .
	manualset3
164915	2	412383	7	NULL	NULL	0	NULL	history	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of history , Epworth Sleepiness Scale Score and body mass index in identifying non-apnoeic snorers .
	manualset3
164916	3	412383	7	NULL	NULL	NULL	NULL	Epworth Sleepiness Scale Score	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The role of history , Epworth Sleepiness Scale Score and body mass index in identifying non-apnoeic snorers .
	manualset3
164917	4	412383	7	NULL	NULL	0	NULL	body mass index	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of history , Epworth Sleepiness Scale Score and body mass index in identifying non-apnoeic snorers .
	manualset3
164918	5	412383	7	NULL	NULL	0	NULL	non-apnoeic snorers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of history , Epworth Sleepiness Scale Score and body mass index in identifying non-apnoeic snorers .
	manualset3
164919	1	412384	7	NULL	NULL	NULL	NULL	 role 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The role of homologous recombination repair ( HRR ) was determined by nuclear Rad51 protein levels and a GFP reporter recombination assay .
	manualset3
164920	2	412384	7	NULL	NULL	0	NULL	homologous recombination repair ( HRR )	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of homologous recombination repair ( HRR ) was determined by nuclear Rad51 protein levels and a GFP reporter recombination assay .
	manualset3
164921	3	412384	7	NULL	NULL	0	NULL	nuclear Rad51 protein levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of homologous recombination repair ( HRR ) was determined by nuclear Rad51 protein levels and a GFP reporter recombination assay .
	manualset3
164922	4	412384	7	NULL	NULL	0	NULL	GFP reporter recombination assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of homologous recombination repair ( HRR ) was determined by nuclear Rad51 protein levels and a GFP reporter recombination assay .
	manualset3
164923	1	412385	7	NULL	NULL	0	NULL	epidemiological studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	According to epidemiological studies , acne is a common condition affecting 80 % of young people between 12 and 18 years of age .
	manualset3
164924	2	412385	7	NULL	NULL	0	NULL	acne	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	According to epidemiological studies , acne is a common condition affecting 80 % of young people between 12 and 18 years of age .
	manualset3
164925	4	412385	7	NULL	NULL	NULL	NULL	80 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	According to epidemiological studies , acne is a common condition affecting 80 % of young people between 12 and 18 years of age .
	manualset3
164926	3	412385	7	NULL	NULL	NULL	NULL	 condition	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	According to epidemiological studies , acne is a common condition affecting 80 % of young people between 12 and 18 years of age .
	manualset3
164927	5	412385	7	NULL	NULL	0	NULL	young people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	According to epidemiological studies , acne is a common condition affecting 80 % of young people between 12 and 18 years of age .
	manualset3
164928	6	412385	7	NULL	NULL	NULL	NULL	12 and 18 years of age	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	According to epidemiological studies , acne is a common condition affecting 80 % of young people between 12 and 18 years of age .
	manualset3
164929	1	412386	7	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of legume and oil seeds in animal nutrition could be more important if negative effects of so-called antinutritional factors ( ANFs ) could be adequately eliminated .
	manualset3
164930	2	412386	7	NULL	NULL	0	NULL	legume	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of legume and oil seeds in animal nutrition could be more important if negative effects of so-called antinutritional factors ( ANFs ) could be adequately eliminated .
	manualset3
164931	3	412386	7	NULL	NULL	0	NULL	oil seeds 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of legume and oil seeds in animal nutrition could be more important if negative effects of so-called antinutritional factors ( ANFs ) could be adequately eliminated .
	manualset3
164932	4	412386	7	NULL	NULL	0	NULL	animal nutrition	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of legume and oil seeds in animal nutrition could be more important if negative effects of so-called antinutritional factors ( ANFs ) could be adequately eliminated .
	manualset3
164933	5	412386	7	NULL	NULL	0	NULL	negative effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of legume and oil seeds in animal nutrition could be more important if negative effects of so-called antinutritional factors ( ANFs ) could be adequately eliminated .
	manualset3
164934	6	412386	7	NULL	NULL	0	NULL	antinutritional factors ( ANFs ) 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of legume and oil seeds in animal nutrition could be more important if negative effects of so-called antinutritional factors ( ANFs ) could be adequately eliminated .
	manualset3
164935	2	412387	7	NULL	NULL	NULL	NULL	maternal syphilis	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The role of maternal syphilis , gonorrhoea and HIV-1 infections in spontaneous abortion .
	manualset3
164936	1	412387	7	NULL	NULL	NULL	NULL	role	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The role of maternal syphilis , gonorrhoea and HIV-1 infections in spontaneous abortion .
	manualset3
164937	3	412387	7	NULL	NULL	0	NULL	 gonorrhoea	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of maternal syphilis , gonorrhoea and HIV-1 infections in spontaneous abortion .
	manualset3
164938	4	412387	7	NULL	NULL	0	NULL	HIV-1 infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of maternal syphilis , gonorrhoea and HIV-1 infections in spontaneous abortion .
	manualset3
164939	5	412387	7	NULL	NULL	0	NULL	spontaneous abortion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of maternal syphilis , gonorrhoea and HIV-1 infections in spontaneous abortion .
	manualset3
164940	1	412388	7	NULL	NULL	NULL	NULL	role	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The role of mitochondrial deficits in ENS neurodegeneration and their relative contribution to gastrointestinal dysfunction , however , are unclear .
	manualset3
164941	2	412388	7	NULL	NULL	0	NULL	mitochondrial deficits	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of mitochondrial deficits in ENS neurodegeneration and their relative contribution to gastrointestinal dysfunction , however , are unclear .
	manualset3
164942	3	412388	7	NULL	NULL	0	NULL	ENS neurodegeneration 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of mitochondrial deficits in ENS neurodegeneration and their relative contribution to gastrointestinal dysfunction , however , are unclear .
	manualset3
164943	4	412388	7	NULL	NULL	0	NULL	contribution	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of mitochondrial deficits in ENS neurodegeneration and their relative contribution to gastrointestinal dysfunction , however , are unclear .
	manualset3
164944	5	412388	7	NULL	NULL	0	NULL	gastrointestinal dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of mitochondrial deficits in ENS neurodegeneration and their relative contribution to gastrointestinal dysfunction , however , are unclear .
	manualset3
164945	1	412389	7	NULL	NULL	0	NULL	 role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of multimodal evoked potentials ( MMEPs ) in establishing multiple sclerosis ( MS ) diagnosis and prognosis has diminished nowadays .
	manualset3
164946	2	412389	7	NULL	NULL	0	NULL	multimodal evoked potentials ( MMEPs )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of multimodal evoked potentials ( MMEPs ) in establishing multiple sclerosis ( MS ) diagnosis and prognosis has diminished nowadays .
	manualset3
164947	3	412389	7	NULL	NULL	0	NULL	multiple sclerosis ( MS ) diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of multimodal evoked potentials ( MMEPs ) in establishing multiple sclerosis ( MS ) diagnosis and prognosis has diminished nowadays .
	manualset3
164948	4	412389	7	NULL	NULL	0	NULL	prognosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of multimodal evoked potentials ( MMEPs ) in establishing multiple sclerosis ( MS ) diagnosis and prognosis has diminished nowadays .
	manualset3
164949	1	412390	7	NULL	NULL	NULL	NULL	role	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The role of nuclear factor NF-Y/CP1 in the transcriptional regulation of the human aldehyde dehydrogenase 2-encoding gene .
	manualset3
164950	2	412390	7	NULL	NULL	0	NULL	 nuclear factor NF-Y/CP1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of nuclear factor NF-Y/CP1 in the transcriptional regulation of the human aldehyde dehydrogenase 2-encoding gene .
	manualset3
164951	3	412390	7	NULL	NULL	0	NULL	transcriptional regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of nuclear factor NF-Y/CP1 in the transcriptional regulation of the human aldehyde dehydrogenase 2-encoding gene .
	manualset3
164952	4	412390	7	NULL	NULL	0	NULL	human aldehyde dehydrogenase 2-encoding gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of nuclear factor NF-Y/CP1 in the transcriptional regulation of the human aldehyde dehydrogenase 2-encoding gene .
	manualset3
164953	1	412391	7	NULL	NULL	0	NULL	 role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of phosphorylated insulin-like growth factor binding protein-1 in predicting pre-term labor in twin pregnancies .
	manualset3
164954	2	412391	7	NULL	NULL	0	NULL	phosphorylated insulin-like growth factor binding protein-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of phosphorylated insulin-like growth factor binding protein-1 in predicting pre-term labor in twin pregnancies .
	manualset3
164955	3	412391	7	NULL	NULL	0	NULL	 pre-term labor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of phosphorylated insulin-like growth factor binding protein-1 in predicting pre-term labor in twin pregnancies .
	manualset3
164956	4	412391	7	NULL	NULL	0	NULL	 twin pregnancies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of phosphorylated insulin-like growth factor binding protein-1 in predicting pre-term labor in twin pregnancies .
	manualset3
164957	1	412392	7	NULL	NULL	0	NULL	 role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of postautograft maintenance remains unclear , but we feel our results are sufficiently encouraging to justify a randomized study , particularly as we studied a group of patients with relatively poor prognoses .
	manualset3
164958	2	412392	7	NULL	NULL	0	NULL	postautograft maintenance	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of postautograft maintenance remains unclear , but we feel our results are sufficiently encouraging to justify a randomized study , particularly as we studied a group of patients with relatively poor prognoses .
	manualset3
164959	3	412392	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of postautograft maintenance remains unclear , but we feel our results are sufficiently encouraging to justify a randomized study , particularly as we studied a group of patients with relatively poor prognoses .
	manualset3
164960	4	412392	7	NULL	NULL	0	NULL	randomized study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of postautograft maintenance remains unclear , but we feel our results are sufficiently encouraging to justify a randomized study , particularly as we studied a group of patients with relatively poor prognoses .
	manualset3
164961	5	412392	7	NULL	NULL	0	NULL	group of patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of postautograft maintenance remains unclear , but we feel our results are sufficiently encouraging to justify a randomized study , particularly as we studied a group of patients with relatively poor prognoses .
	manualset3
164962	6	412392	7	NULL	NULL	0	NULL	poor prognoses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of postautograft maintenance remains unclear , but we feel our results are sufficiently encouraging to justify a randomized study , particularly as we studied a group of patients with relatively poor prognoses .
	manualset3
164963	1	412393	7	NULL	NULL	NULL	NULL	role	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The role of region I , a transcriptional enhancer in cells that express EBNA-1 , in replication is not understood .
	manualset3
164964	2	412393	7	NULL	NULL	0	NULL	 region I	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of region I , a transcriptional enhancer in cells that express EBNA-1 , in replication is not understood .
	manualset3
164965	3	412393	7	NULL	NULL	0	NULL	transcriptional enhancer	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of region I , a transcriptional enhancer in cells that express EBNA-1 , in replication is not understood .
	manualset3
164966	4	412393	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of region I , a transcriptional enhancer in cells that express EBNA-1 , in replication is not understood .
	manualset3
164967	5	412393	7	NULL	NULL	0	NULL	EBNA-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of region I , a transcriptional enhancer in cells that express EBNA-1 , in replication is not understood .
	manualset3
164968	6	412393	7	NULL	NULL	0	NULL	replication 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of region I , a transcriptional enhancer in cells that express EBNA-1 , in replication is not understood .
	manualset3
164969	1	412394	7	NULL	NULL	0	NULL	role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of respiratory viruses in predisposing to colonization and invasion of bacterial organisms has often been suggested .
	manualset3
164970	2	412394	7	NULL	NULL	0	NULL	respiratory viruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of respiratory viruses in predisposing to colonization and invasion of bacterial organisms has often been suggested .
	manualset3
164971	3	412394	7	NULL	NULL	0	NULL	colonization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of respiratory viruses in predisposing to colonization and invasion of bacterial organisms has often been suggested .
	manualset3
164972	4	412394	7	NULL	NULL	0	NULL	invasion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of respiratory viruses in predisposing to colonization and invasion of bacterial organisms has often been suggested .
	manualset3
164973	5	412394	7	NULL	NULL	0	NULL	bacterial organisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of respiratory viruses in predisposing to colonization and invasion of bacterial organisms has often been suggested .
	manualset3
164974	1	412395	7	NULL	NULL	0	NULL	role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of senescence in the action of antitumor drugs .
	manualset3
164975	2	412395	7	NULL	NULL	0	NULL	 senescence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of senescence in the action of antitumor drugs .
	manualset3
164976	3	412395	7	NULL	NULL	NULL	NULL	action	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The role of senescence in the action of antitumor drugs .
	manualset3
164977	4	412395	7	NULL	NULL	0	NULL	antitumor drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of senescence in the action of antitumor drugs .
	manualset3
164978	1	412396	7	NULL	NULL	0	NULL	model-building techniques	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	According to model-building techniques and energy calculations , a total of seven molecular structures ( three with C2 ' - endo and four with C3 ' - endo sugars ) , all of pitch 8.74 A , and hence seven different crystal-packing arrangements are the most probable .
	manualset3
164979	2	412396	7	NULL	NULL	0	NULL	energy calculations	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	According to model-building techniques and energy calculations , a total of seven molecular structures ( three with C2 ' - endo and four with C3 ' - endo sugars ) , all of pitch 8.74 A , and hence seven different crystal-packing arrangements are the most probable .
	manualset3
164980	3	412396	7	NULL	NULL	0	NULL	total	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	According to model-building techniques and energy calculations , a total of seven molecular structures ( three with C2 ' - endo and four with C3 ' - endo sugars ) , all of pitch 8.74 A , and hence seven different crystal-packing arrangements are the most probable .
	manualset3
164981	4	412396	7	NULL	NULL	0	NULL	seven molecular structures 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	According to model-building techniques and energy calculations , a total of seven molecular structures ( three with C2 ' - endo and four with C3 ' - endo sugars ) , all of pitch 8.74 A , and hence seven different crystal-packing arrangements are the most probable .
	manualset3
164982	5	412396	7	NULL	NULL	0	NULL	three with C2 ' - endo and four with C3 ' - endo sugars 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	According to model-building techniques and energy calculations , a total of seven molecular structures ( three with C2 ' - endo and four with C3 ' - endo sugars ) , all of pitch 8.74 A , and hence seven different crystal-packing arrangements are the most probable .
	manualset3
164983	6	412396	7	NULL	NULL	0	NULL	pitch 8.74 A	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	According to model-building techniques and energy calculations , a total of seven molecular structures ( three with C2 ' - endo and four with C3 ' - endo sugars ) , all of pitch 8.74 A , and hence seven different crystal-packing arrangements are the most probable .
	manualset3
164984	7	412396	7	NULL	NULL	0	NULL	seven different crystal-packing arrangements	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	According to model-building techniques and energy calculations , a total of seven molecular structures ( three with C2 ' - endo and four with C3 ' - endo sugars ) , all of pitch 8.74 A , and hence seven different crystal-packing arrangements are the most probable .
	manualset3
164985	1	412397	7	NULL	NULL	0	NULL	 role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of serology in infectious disease diagnosis is highlighted by HIV and viral hepatitis diagnosis developed since the 80 's .
	manualset3
164986	2	412397	7	NULL	NULL	0	NULL	serology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of serology in infectious disease diagnosis is highlighted by HIV and viral hepatitis diagnosis developed since the 80 's .
	manualset3
164987	3	412397	7	NULL	NULL	0	NULL	 infectious disease diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of serology in infectious disease diagnosis is highlighted by HIV and viral hepatitis diagnosis developed since the 80 's .
	manualset3
164988	4	412397	7	NULL	NULL	0	NULL	HIV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of serology in infectious disease diagnosis is highlighted by HIV and viral hepatitis diagnosis developed since the 80 's .
	manualset3
164989	5	412397	7	NULL	NULL	0	NULL	viral hepatitis diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of serology in infectious disease diagnosis is highlighted by HIV and viral hepatitis diagnosis developed since the 80 's .
	manualset3
164990	6	412397	7	NULL	NULL	0	NULL	80 's	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of serology in infectious disease diagnosis is highlighted by HIV and viral hepatitis diagnosis developed since the 80 's .
	manualset3
164991	1	412398	7	NULL	NULL	0	NULL	 role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of starch in renal dysfunction , the importance of the definition of acute kidney injury and acute renal failure , and hyperoncoticity are reviewed .
	manualset3
164992	2	412398	7	NULL	NULL	0	NULL	 starch	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of starch in renal dysfunction , the importance of the definition of acute kidney injury and acute renal failure , and hyperoncoticity are reviewed .
	manualset3
164993	3	412398	7	NULL	NULL	0	NULL	renal dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of starch in renal dysfunction , the importance of the definition of acute kidney injury and acute renal failure , and hyperoncoticity are reviewed .
	manualset3
164995	4	412398	7	NULL	NULL	NULL	NULL	definition	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The role of starch in renal dysfunction , the importance of the definition of acute kidney injury and acute renal failure , and hyperoncoticity are reviewed .
	manualset3
164996	5	412398	7	NULL	NULL	0	NULL	acute kidney injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of starch in renal dysfunction , the importance of the definition of acute kidney injury and acute renal failure , and hyperoncoticity are reviewed .
	manualset3
164997	6	412398	7	NULL	NULL	0	NULL	acute renal failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of starch in renal dysfunction , the importance of the definition of acute kidney injury and acute renal failure , and hyperoncoticity are reviewed .
	manualset3
164998	7	412398	7	NULL	NULL	0	NULL	hyperoncoticity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of starch in renal dysfunction , the importance of the definition of acute kidney injury and acute renal failure , and hyperoncoticity are reviewed .
	manualset3
164999	1	412399	7	NULL	NULL	NULL	NULL	role	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The role of subunit hinges and molecular `` switches '' in the control of viral capsid polymorphism .
	manualset3
165000	2	412399	7	NULL	NULL	0	NULL	subunit hinges 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of subunit hinges and molecular `` switches '' in the control of viral capsid polymorphism .
	manualset3
165001	3	412399	7	NULL	NULL	0	NULL	molecular `` switches '' 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of subunit hinges and molecular `` switches '' in the control of viral capsid polymorphism .
	manualset3
165002	4	412399	7	NULL	NULL	0	NULL	control	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of subunit hinges and molecular `` switches '' in the control of viral capsid polymorphism .
	manualset3
165003	5	412399	7	NULL	NULL	0	NULL	viral capsid polymorphism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of subunit hinges and molecular `` switches '' in the control of viral capsid polymorphism .
	manualset3
165004	1	412400	7	NULL	NULL	NULL	NULL	role	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The role of synaptic vesicles .
	manualset3
165005	2	412400	7	NULL	NULL	0	NULL	synaptic vesicles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of synaptic vesicles .
	manualset3
165007	1	412401	7	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of synchronization of information processes in the mechanisms of short-term memory and the involvement of the cholinergic and glutaminergic systems are discussed .
	manualset3
165008	2	412401	7	NULL	NULL	0	NULL	synchronization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of synchronization of information processes in the mechanisms of short-term memory and the involvement of the cholinergic and glutaminergic systems are discussed .
	manualset3
165009	3	412401	7	NULL	NULL	0	NULL	information processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of synchronization of information processes in the mechanisms of short-term memory and the involvement of the cholinergic and glutaminergic systems are discussed .
	manualset3
165010	4	412401	7	NULL	NULL	0	NULL	mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of synchronization of information processes in the mechanisms of short-term memory and the involvement of the cholinergic and glutaminergic systems are discussed .
	manualset3
165011	5	412401	7	NULL	NULL	0	NULL	short-term memory	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of synchronization of information processes in the mechanisms of short-term memory and the involvement of the cholinergic and glutaminergic systems are discussed .
	manualset3
165012	6	412401	7	NULL	NULL	0	NULL	involvement 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of synchronization of information processes in the mechanisms of short-term memory and the involvement of the cholinergic and glutaminergic systems are discussed .
	manualset3
165013	7	412401	7	NULL	NULL	0	NULL	cholinergic systems	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of synchronization of information processes in the mechanisms of short-term memory and the involvement of the cholinergic and glutaminergic systems are discussed .
	manualset3
165014	8	412401	7	NULL	NULL	0	NULL	glutaminergic systems 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of synchronization of information processes in the mechanisms of short-term memory and the involvement of the cholinergic and glutaminergic systems are discussed .
	manualset3
165015	1	412402	7	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of the bisecting GlcNAc residue in affecting the binding properties of complex type carbohydrates to ConA is discussed , and the results are related to the possible structure-function properties of complex type glycopeptides on the surface of cells .
	manualset3
165016	2	412402	7	NULL	NULL	0	NULL	bisecting GlcNAc residue	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of the bisecting GlcNAc residue in affecting the binding properties of complex type carbohydrates to ConA is discussed , and the results are related to the possible structure-function properties of complex type glycopeptides on the surface of cells .
	manualset3
165017	3	412402	7	NULL	NULL	NULL	NULL	 binding properties	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The role of the bisecting GlcNAc residue in affecting the binding properties of complex type carbohydrates to ConA is discussed , and the results are related to the possible structure-function properties of complex type glycopeptides on the surface of cells .
	manualset3
165018	4	412402	7	NULL	NULL	0	NULL	complex type carbohydrates	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of the bisecting GlcNAc residue in affecting the binding properties of complex type carbohydrates to ConA is discussed , and the results are related to the possible structure-function properties of complex type glycopeptides on the surface of cells .
	manualset3
165019	5	412402	7	NULL	NULL	0	NULL	ConA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of the bisecting GlcNAc residue in affecting the binding properties of complex type carbohydrates to ConA is discussed , and the results are related to the possible structure-function properties of complex type glycopeptides on the surface of cells .
	manualset3
165020	6	412402	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of the bisecting GlcNAc residue in affecting the binding properties of complex type carbohydrates to ConA is discussed , and the results are related to the possible structure-function properties of complex type glycopeptides on the surface of cells .
	manualset3
165021	7	412402	7	NULL	NULL	0	NULL	structure-function properties 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of the bisecting GlcNAc residue in affecting the binding properties of complex type carbohydrates to ConA is discussed , and the results are related to the possible structure-function properties of complex type glycopeptides on the surface of cells .
	manualset3
165022	8	412402	7	NULL	NULL	0	NULL	complex type glycopeptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of the bisecting GlcNAc residue in affecting the binding properties of complex type carbohydrates to ConA is discussed , and the results are related to the possible structure-function properties of complex type glycopeptides on the surface of cells .
	manualset3
165023	9	412402	7	NULL	NULL	0	NULL	surface of cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of the bisecting GlcNAc residue in affecting the binding properties of complex type carbohydrates to ConA is discussed , and the results are related to the possible structure-function properties of complex type glycopeptides on the surface of cells .
	manualset3
165024	1	412403	7	NULL	NULL	0	NULL	role 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of the emergency physician in the management of Jehovah 's Witnesses .
	manualset3
165025	2	412403	7	NULL	NULL	0	NULL	emergency physician	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of the emergency physician in the management of Jehovah 's Witnesses .
	manualset3
165026	3	412403	7	NULL	NULL	0	NULL	management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of the emergency physician in the management of Jehovah 's Witnesses .
	manualset3
165027	4	412403	7	NULL	NULL	0	NULL	Jehovah 's Witnesses	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of the emergency physician in the management of Jehovah 's Witnesses .
	manualset3
165028	1	412404	7	NULL	NULL	0	NULL	role 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of the endothelium in response to aggregating platelets was examined in porcine coronary and peripheral ( carotid , femoral and renal ) arteries from normal and hypercholesterolemic pigs .
	manualset3
165029	2	412404	7	NULL	NULL	NULL	NULL	endothelium	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The role of the endothelium in response to aggregating platelets was examined in porcine coronary and peripheral ( carotid , femoral and renal ) arteries from normal and hypercholesterolemic pigs .
	manualset3
165030	3	412404	7	NULL	NULL	0	NULL	aggregating platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of the endothelium in response to aggregating platelets was examined in porcine coronary and peripheral ( carotid , femoral and renal ) arteries from normal and hypercholesterolemic pigs .
	manualset3
165031	4	412404	7	NULL	NULL	0	NULL	porcine coronary arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of the endothelium in response to aggregating platelets was examined in porcine coronary and peripheral ( carotid , femoral and renal ) arteries from normal and hypercholesterolemic pigs .
	manualset3
165032	5	412404	7	NULL	NULL	0	NULL	 peripheral  arteries 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of the endothelium in response to aggregating platelets was examined in porcine coronary and peripheral ( carotid , femoral and renal ) arteries from normal and hypercholesterolemic pigs .
	manualset3
165033	6	412404	7	NULL	NULL	0	NULL	carotid arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of the endothelium in response to aggregating platelets was examined in porcine coronary and peripheral ( carotid , femoral and renal ) arteries from normal and hypercholesterolemic pigs .
	manualset3
165034	7	412404	7	NULL	NULL	0	NULL	femoral arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of the endothelium in response to aggregating platelets was examined in porcine coronary and peripheral ( carotid , femoral and renal ) arteries from normal and hypercholesterolemic pigs .
	manualset3
165035	8	412404	7	NULL	NULL	0	NULL	renal  arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of the endothelium in response to aggregating platelets was examined in porcine coronary and peripheral ( carotid , femoral and renal ) arteries from normal and hypercholesterolemic pigs .
	manualset3
165036	9	412404	7	NULL	NULL	0	NULL	normal pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of the endothelium in response to aggregating platelets was examined in porcine coronary and peripheral ( carotid , femoral and renal ) arteries from normal and hypercholesterolemic pigs .
	manualset3
165037	10	412404	7	NULL	NULL	0	NULL	hypercholesterolemic pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of the endothelium in response to aggregating platelets was examined in porcine coronary and peripheral ( carotid , femoral and renal ) arteries from normal and hypercholesterolemic pigs .
	manualset3
165038	1	412405	7	NULL	NULL	0	NULL	role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of the health care professions in preventing surgical site infection .
	manualset3
165039	2	412405	7	NULL	NULL	NULL	NULL	health care professions	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The role of the health care professions in preventing surgical site infection .
	manualset3
165040	3	412405	7	NULL	NULL	0	NULL	surgical site infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of the health care professions in preventing surgical site infection .
	manualset3
165041	1	412406	7	NULL	NULL	NULL	NULL	multivariate regression analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	According to multivariate regression analysis , the significant factors associated with improvement in walking capacity during this period were an unstable fracture type ( p = 0.003 ) , improvement of hip strength ( p = 0.006 ) , and improvement of pain ( p = 0.03 ) .
	manualset3
165042	2	412406	7	NULL	NULL	0	NULL	factors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	According to multivariate regression analysis , the significant factors associated with improvement in walking capacity during this period were an unstable fracture type ( p = 0.003 ) , improvement of hip strength ( p = 0.006 ) , and improvement of pain ( p = 0.03 ) .
	manualset3
165043	3	412406	7	NULL	NULL	0	NULL	walking capacity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	According to multivariate regression analysis , the significant factors associated with improvement in walking capacity during this period were an unstable fracture type ( p = 0.003 ) , improvement of hip strength ( p = 0.006 ) , and improvement of pain ( p = 0.03 ) .
	manualset3
165044	4	412406	7	NULL	NULL	0	NULL	period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	According to multivariate regression analysis , the significant factors associated with improvement in walking capacity during this period were an unstable fracture type ( p = 0.003 ) , improvement of hip strength ( p = 0.006 ) , and improvement of pain ( p = 0.03 ) .
	manualset3
165045	5	412406	7	NULL	NULL	0	NULL	unstable fracture type	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	According to multivariate regression analysis , the significant factors associated with improvement in walking capacity during this period were an unstable fracture type ( p = 0.003 ) , improvement of hip strength ( p = 0.006 ) , and improvement of pain ( p = 0.03 ) .
	manualset3
165046	6	412406	7	NULL	NULL	0	NULL	p = 0.003	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	According to multivariate regression analysis , the significant factors associated with improvement in walking capacity during this period were an unstable fracture type ( p = 0.003 ) , improvement of hip strength ( p = 0.006 ) , and improvement of pain ( p = 0.03 ) .
	manualset3
165047	7	412406	7	NULL	NULL	0	NULL	improvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	According to multivariate regression analysis , the significant factors associated with improvement in walking capacity during this period were an unstable fracture type ( p = 0.003 ) , improvement of hip strength ( p = 0.006 ) , and improvement of pain ( p = 0.03 ) .
	manualset3
165048	8	412406	7	NULL	NULL	0	NULL	hip strength	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	According to multivariate regression analysis , the significant factors associated with improvement in walking capacity during this period were an unstable fracture type ( p = 0.003 ) , improvement of hip strength ( p = 0.006 ) , and improvement of pain ( p = 0.03 ) .
	manualset3
165049	9	412406	7	NULL	NULL	0	NULL	p = 0.006	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	According to multivariate regression analysis , the significant factors associated with improvement in walking capacity during this period were an unstable fracture type ( p = 0.003 ) , improvement of hip strength ( p = 0.006 ) , and improvement of pain ( p = 0.03 ) .
	manualset3
165050	10	412406	7	NULL	NULL	0	NULL	 improvement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	According to multivariate regression analysis , the significant factors associated with improvement in walking capacity during this period were an unstable fracture type ( p = 0.003 ) , improvement of hip strength ( p = 0.006 ) , and improvement of pain ( p = 0.03 ) .
	manualset3
165051	11	412406	7	NULL	NULL	0	NULL	pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	According to multivariate regression analysis , the significant factors associated with improvement in walking capacity during this period were an unstable fracture type ( p = 0.003 ) , improvement of hip strength ( p = 0.006 ) , and improvement of pain ( p = 0.03 ) .
	manualset3
165052	12	412406	7	NULL	NULL	0	NULL	p = 0.03	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	According to multivariate regression analysis , the significant factors associated with improvement in walking capacity during this period were an unstable fracture type ( p = 0.003 ) , improvement of hip strength ( p = 0.006 ) , and improvement of pain ( p = 0.03 ) .
	manualset3
165053	1	412407	7	NULL	NULL	0	NULL	 role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of the homeobox gene HOXA5 in normal human hematopoiesis was studied by constitutively expressing the HOXA5 cDNA in CD34 ( + ) and CD34 ( + ) CD38 ( - ) cells from bone marrow and cord blood .
	manualset3
165054	2	412407	7	NULL	NULL	0	NULL	 homeobox gene HOXA5	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of the homeobox gene HOXA5 in normal human hematopoiesis was studied by constitutively expressing the HOXA5 cDNA in CD34 ( + ) and CD34 ( + ) CD38 ( - ) cells from bone marrow and cord blood .
	manualset3
165055	3	412407	7	NULL	NULL	0	NULL	normal human hematopoiesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of the homeobox gene HOXA5 in normal human hematopoiesis was studied by constitutively expressing the HOXA5 cDNA in CD34 ( + ) and CD34 ( + ) CD38 ( - ) cells from bone marrow and cord blood .
	manualset3
165056	4	412407	7	NULL	NULL	NULL	NULL	HOXA5 cDNA	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The role of the homeobox gene HOXA5 in normal human hematopoiesis was studied by constitutively expressing the HOXA5 cDNA in CD34 ( + ) and CD34 ( + ) CD38 ( - ) cells from bone marrow and cord blood .
	manualset3
165057	5	412407	7	NULL	NULL	0	NULL	CD34 ( + ) cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of the homeobox gene HOXA5 in normal human hematopoiesis was studied by constitutively expressing the HOXA5 cDNA in CD34 ( + ) and CD34 ( + ) CD38 ( - ) cells from bone marrow and cord blood .
	manualset3
165058	6	412407	7	NULL	NULL	NULL	NULL	CD34 ( + ) CD38 ( - ) cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The role of the homeobox gene HOXA5 in normal human hematopoiesis was studied by constitutively expressing the HOXA5 cDNA in CD34 ( + ) and CD34 ( + ) CD38 ( - ) cells from bone marrow and cord blood .
	manualset3
165060	7	412407	7	NULL	NULL	NULL	NULL	bone marrow	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The role of the homeobox gene HOXA5 in normal human hematopoiesis was studied by constitutively expressing the HOXA5 cDNA in CD34 ( + ) and CD34 ( + ) CD38 ( - ) cells from bone marrow and cord blood .
	manualset3
165061	8	412407	7	NULL	NULL	NULL	NULL	cord blood	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The role of the homeobox gene HOXA5 in normal human hematopoiesis was studied by constitutively expressing the HOXA5 cDNA in CD34 ( + ) and CD34 ( + ) CD38 ( - ) cells from bone marrow and cord blood .
	manualset3
165062	1	412408	7	NULL	NULL	0	NULL	roles	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The roles of K-ras in neoplasia are not entirely understood , although there is evidence that K-ras affects susceptibility to apoptosis , modulating survival of DNA damaged cells which would otherwise be eliminated .
	manualset3
165063	2	412408	7	NULL	NULL	0	NULL	K-ras	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The roles of K-ras in neoplasia are not entirely understood , although there is evidence that K-ras affects susceptibility to apoptosis , modulating survival of DNA damaged cells which would otherwise be eliminated .
	manualset3
165064	3	412408	7	NULL	NULL	0	NULL	neoplasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The roles of K-ras in neoplasia are not entirely understood , although there is evidence that K-ras affects susceptibility to apoptosis , modulating survival of DNA damaged cells which would otherwise be eliminated .
	manualset3
165065	4	412408	7	NULL	NULL	0	NULL	K-ras	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The roles of K-ras in neoplasia are not entirely understood , although there is evidence that K-ras affects susceptibility to apoptosis , modulating survival of DNA damaged cells which would otherwise be eliminated .
	manualset3
165066	5	412408	7	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The roles of K-ras in neoplasia are not entirely understood , although there is evidence that K-ras affects susceptibility to apoptosis , modulating survival of DNA damaged cells which would otherwise be eliminated .
	manualset3
165067	6	412408	7	NULL	NULL	NULL	NULL	 DNA damaged cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The roles of K-ras in neoplasia are not entirely understood , although there is evidence that K-ras affects susceptibility to apoptosis , modulating survival of DNA damaged cells which would otherwise be eliminated .
	manualset3
165872	7	412408	7	NULL	NULL	0	NULL	survival	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The roles of K-ras in neoplasia are not entirely understood , although there is evidence that K-ras affects susceptibility to apoptosis , modulating survival of DNA damaged cells which would otherwise be eliminated .
	manualset3
166496	8	412408	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The roles of K-ras in neoplasia are not entirely understood , although there is evidence that K-ras affects susceptibility to apoptosis , modulating survival of DNA damaged cells which would otherwise be eliminated .
	manualset3
166497	9	412408	7	NULL	NULL	0	NULL	susceptibility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The roles of K-ras in neoplasia are not entirely understood , although there is evidence that K-ras affects susceptibility to apoptosis , modulating survival of DNA damaged cells which would otherwise be eliminated .
	manualset3
165068	1	412409	7	NULL	NULL	0	NULL	 roles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The roles of academia , health authorities and government are presently unclear , with leadership differences , power discrepancies , conflicting agendas , lag times and systemic structural complexity .
	manualset3
165069	2	412409	7	NULL	NULL	0	NULL	academia	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The roles of academia , health authorities and government are presently unclear , with leadership differences , power discrepancies , conflicting agendas , lag times and systemic structural complexity .
	manualset3
165070	3	412409	7	NULL	NULL	0	NULL	health authorities	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The roles of academia , health authorities and government are presently unclear , with leadership differences , power discrepancies , conflicting agendas , lag times and systemic structural complexity .
	manualset3
165071	4	412409	7	NULL	NULL	0	NULL	government	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The roles of academia , health authorities and government are presently unclear , with leadership differences , power discrepancies , conflicting agendas , lag times and systemic structural complexity .
	manualset3
165072	5	412409	7	NULL	NULL	NULL	NULL	leadership differences	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The roles of academia , health authorities and government are presently unclear , with leadership differences , power discrepancies , conflicting agendas , lag times and systemic structural complexity .
	manualset3
165073	6	412409	7	NULL	NULL	0	NULL	power discrepancies 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The roles of academia , health authorities and government are presently unclear , with leadership differences , power discrepancies , conflicting agendas , lag times and systemic structural complexity .
	manualset3
165074	7	412409	7	NULL	NULL	0	NULL	conflicting agendas	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The roles of academia , health authorities and government are presently unclear , with leadership differences , power discrepancies , conflicting agendas , lag times and systemic structural complexity .
	manualset3
165075	8	412409	7	NULL	NULL	0	NULL	lag times	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The roles of academia , health authorities and government are presently unclear , with leadership differences , power discrepancies , conflicting agendas , lag times and systemic structural complexity .
	manualset3
165076	9	412409	7	NULL	NULL	0	NULL	systemic structural complexity 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The roles of academia , health authorities and government are presently unclear , with leadership differences , power discrepancies , conflicting agendas , lag times and systemic structural complexity .
	manualset3
165077	1	412410	7	NULL	NULL	0	NULL	roles	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The roles of these hormones in the primary culture of isolated hepatic cells are discussed in the present paper .
	manualset3
165078	2	412410	7	NULL	NULL	NULL	NULL	hormones	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The roles of these hormones in the primary culture of isolated hepatic cells are discussed in the present paper .
	manualset3
165079	3	412410	7	NULL	NULL	0	NULL	 primary culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The roles of these hormones in the primary culture of isolated hepatic cells are discussed in the present paper .
	manualset3
165080	4	412410	7	NULL	NULL	0	NULL	isolated hepatic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The roles of these hormones in the primary culture of isolated hepatic cells are discussed in the present paper .
	manualset3
165081	5	412410	7	NULL	NULL	0	NULL	paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The roles of these hormones in the primary culture of isolated hepatic cells are discussed in the present paper .
	manualset3
165082	1	412411	7	NULL	NULL	0	NULL	round migrating cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The round migrating cells are classified as retinal progenitor cells since they immunostained for opsin and interphotoreceptor retinoid-binding protein ( IRBP ) , two photoreceptor cell markers , and a few for cellular retinaldehyde binding protein ( CRALBP ) , a Muller cell marker .
	manualset3
165083	2	412411	7	NULL	NULL	0	NULL	retinal progenitor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The round migrating cells are classified as retinal progenitor cells since they immunostained for opsin and interphotoreceptor retinoid-binding protein ( IRBP ) , two photoreceptor cell markers , and a few for cellular retinaldehyde binding protein ( CRALBP ) , a Muller cell marker .
	manualset3
165084	3	412411	7	NULL	NULL	0	NULL	opsin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The round migrating cells are classified as retinal progenitor cells since they immunostained for opsin and interphotoreceptor retinoid-binding protein ( IRBP ) , two photoreceptor cell markers , and a few for cellular retinaldehyde binding protein ( CRALBP ) , a Muller cell marker .
	manualset3
165085	4	412411	7	NULL	NULL	0	NULL	interphotoreceptor retinoid-binding protein ( IRBP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The round migrating cells are classified as retinal progenitor cells since they immunostained for opsin and interphotoreceptor retinoid-binding protein ( IRBP ) , two photoreceptor cell markers , and a few for cellular retinaldehyde binding protein ( CRALBP ) , a Muller cell marker .
	manualset3
165086	5	412411	7	NULL	NULL	NULL	NULL	two photoreceptor cell markers	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The round migrating cells are classified as retinal progenitor cells since they immunostained for opsin and interphotoreceptor retinoid-binding protein ( IRBP ) , two photoreceptor cell markers , and a few for cellular retinaldehyde binding protein ( CRALBP ) , a Muller cell marker .
	manualset3
165087	6	412411	7	NULL	NULL	0	NULL	cellular retinaldehyde binding protein ( CRALBP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The round migrating cells are classified as retinal progenitor cells since they immunostained for opsin and interphotoreceptor retinoid-binding protein ( IRBP ) , two photoreceptor cell markers , and a few for cellular retinaldehyde binding protein ( CRALBP ) , a Muller cell marker .
	manualset3
165088	7	412411	7	NULL	NULL	0	NULL	Muller cell marker	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The round migrating cells are classified as retinal progenitor cells since they immunostained for opsin and interphotoreceptor retinoid-binding protein ( IRBP ) , two photoreceptor cell markers , and a few for cellular retinaldehyde binding protein ( CRALBP ) , a Muller cell marker .
	manualset3
165089	1	412412	7	NULL	NULL	0	NULL	 rudiments 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The rudiments of programming in BASIC for the BBC microcomputer are outlined .
	manualset3
165090	2	412412	7	NULL	NULL	0	NULL	programming 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The rudiments of programming in BASIC for the BBC microcomputer are outlined .
	manualset3
165091	3	412412	7	NULL	NULL	0	NULL	BASIC	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The rudiments of programming in BASIC for the BBC microcomputer are outlined .
	manualset3
165092	4	412412	7	NULL	NULL	NULL	NULL	BBC microcomputer 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The rudiments of programming in BASIC for the BBC microcomputer are outlined .
	manualset3
165093	1	412413	7	NULL	NULL	0	NULL	run-down	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The run-down of the GABAA response was reversed when Mg2 + ( 4 mM ) and ATP ( 2 mM ) were introduced into the intracellular perfusate .
	manualset3
165094	2	412413	7	NULL	NULL	0	NULL	GABAA response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The run-down of the GABAA response was reversed when Mg2 + ( 4 mM ) and ATP ( 2 mM ) were introduced into the intracellular perfusate .
	manualset3
165095	3	412413	7	NULL	NULL	0	NULL	 Mg2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The run-down of the GABAA response was reversed when Mg2 + ( 4 mM ) and ATP ( 2 mM ) were introduced into the intracellular perfusate .
	manualset3
165096	4	412413	7	NULL	NULL	0	NULL	 4 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The run-down of the GABAA response was reversed when Mg2 + ( 4 mM ) and ATP ( 2 mM ) were introduced into the intracellular perfusate .
	manualset3
165097	5	412413	7	NULL	NULL	0	NULL	ATP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The run-down of the GABAA response was reversed when Mg2 + ( 4 mM ) and ATP ( 2 mM ) were introduced into the intracellular perfusate .
	manualset3
165098	6	412413	7	NULL	NULL	0	NULL	2 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The run-down of the GABAA response was reversed when Mg2 + ( 4 mM ) and ATP ( 2 mM ) were introduced into the intracellular perfusate .
	manualset3
165099	7	412413	7	NULL	NULL	0	NULL	intracellular perfusate	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The run-down of the GABAA response was reversed when Mg2 + ( 4 mM ) and ATP ( 2 mM ) were introduced into the intracellular perfusate .
	manualset3
165100	1	412414	7	NULL	NULL	0	NULL	Clinico-laboratory characteristics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinico-laboratory characteristics and treatment of patients with trichinosis ) .
	manualset3
165101	2	412414	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinico-laboratory characteristics and treatment of patients with trichinosis ) .
	manualset3
165102	3	412414	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinico-laboratory characteristics and treatment of patients with trichinosis ) .
	manualset3
165103	4	412414	7	NULL	NULL	0	NULL	trichinosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinico-laboratory characteristics and treatment of patients with trichinosis ) .
	manualset3
165104	1	412415	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our data , the number of dialysis did not play any role in the frequency of infections .
	manualset3
165105	2	412415	7	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our data , the number of dialysis did not play any role in the frequency of infections .
	manualset3
165106	3	412415	7	NULL	NULL	0	NULL	dialysis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our data , the number of dialysis did not play any role in the frequency of infections .
	manualset3
165107	4	412415	7	NULL	NULL	0	NULL	role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our data , the number of dialysis did not play any role in the frequency of infections .
	manualset3
165108	5	412415	7	NULL	NULL	0	NULL	frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our data , the number of dialysis did not play any role in the frequency of infections .
	manualset3
165109	6	412415	7	NULL	NULL	0	NULL	infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our data , the number of dialysis did not play any role in the frequency of infections .
	manualset3
165110	1	412416	7	NULL	NULL	0	NULL	TP concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The runoff TP concentration was higher in bamboo timber forest than in bamboo shoot forest , but the TP loss from the sediment runoff in bamboo shoot forest was hundreds times of that in bamboo timber forest .
	manualset3
165111	2	412416	7	NULL	NULL	NULL	NULL	bamboo timber forest	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The runoff TP concentration was higher in bamboo timber forest than in bamboo shoot forest , but the TP loss from the sediment runoff in bamboo shoot forest was hundreds times of that in bamboo timber forest .
	manualset3
165112	3	412416	7	NULL	NULL	NULL	NULL	bamboo shoot forest	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The runoff TP concentration was higher in bamboo timber forest than in bamboo shoot forest , but the TP loss from the sediment runoff in bamboo shoot forest was hundreds times of that in bamboo timber forest .
	manualset3
165113	4	412416	7	NULL	NULL	0	NULL	TP loss	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The runoff TP concentration was higher in bamboo timber forest than in bamboo shoot forest , but the TP loss from the sediment runoff in bamboo shoot forest was hundreds times of that in bamboo timber forest .
	manualset3
165114	5	412416	7	NULL	NULL	0	NULL	sediment	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The runoff TP concentration was higher in bamboo timber forest than in bamboo shoot forest , but the TP loss from the sediment runoff in bamboo shoot forest was hundreds times of that in bamboo timber forest .
	manualset3
165115	6	412416	7	NULL	NULL	NULL	NULL	bamboo shoot forest	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The runoff TP concentration was higher in bamboo timber forest than in bamboo shoot forest , but the TP loss from the sediment runoff in bamboo shoot forest was hundreds times of that in bamboo timber forest .
	manualset3
165116	7	412416	7	NULL	NULL	0	NULL	hundreds times	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The runoff TP concentration was higher in bamboo timber forest than in bamboo shoot forest , but the TP loss from the sediment runoff in bamboo shoot forest was hundreds times of that in bamboo timber forest .
	manualset3
165117	8	412416	7	NULL	NULL	NULL	NULL	bamboo timber forest	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The runoff TP concentration was higher in bamboo timber forest than in bamboo shoot forest , but the TP loss from the sediment runoff in bamboo shoot forest was hundreds times of that in bamboo timber forest .
	manualset3
165118	1	412417	7	NULL	NULL	0	NULL	runt-related transcription factor 1 RUNX1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The runt-related transcription factor 1 , RUNX1 , is crucial in the development of myeloid and lymphoid cell lineages and has been reported to be mutated in myeloid malignancies in approximately 30 % of cases .
	manualset3
165119	2	412417	7	NULL	NULL	0	NULL	 development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The runt-related transcription factor 1 , RUNX1 , is crucial in the development of myeloid and lymphoid cell lineages and has been reported to be mutated in myeloid malignancies in approximately 30 % of cases .
	manualset3
165120	3	412417	7	NULL	NULL	0	NULL	myeloid cell lineages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The runt-related transcription factor 1 , RUNX1 , is crucial in the development of myeloid and lymphoid cell lineages and has been reported to be mutated in myeloid malignancies in approximately 30 % of cases .
	manualset3
165121	4	412417	7	NULL	NULL	0	NULL	lymphoid cell lineages 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The runt-related transcription factor 1 , RUNX1 , is crucial in the development of myeloid and lymphoid cell lineages and has been reported to be mutated in myeloid malignancies in approximately 30 % of cases .
	manualset3
165122	5	412417	7	NULL	NULL	0	NULL	myeloid malignancies	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The runt-related transcription factor 1 , RUNX1 , is crucial in the development of myeloid and lymphoid cell lineages and has been reported to be mutated in myeloid malignancies in approximately 30 % of cases .
	manualset3
165123	6	412417	7	NULL	NULL	0	NULL	30 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The runt-related transcription factor 1 , RUNX1 , is crucial in the development of myeloid and lymphoid cell lineages and has been reported to be mutated in myeloid malignancies in approximately 30 % of cases .
	manualset3
165124	7	412417	7	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The runt-related transcription factor 1 , RUNX1 , is crucial in the development of myeloid and lymphoid cell lineages and has been reported to be mutated in myeloid malignancies in approximately 30 % of cases .
	manualset3
165125	1	412418	7	NULL	NULL	0	NULL	safety	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The safety and effectiveness of systemic and topical medical therapies for ocular disorders are limited due to poor ocular drug uptake , nonspecificity to target tissues , systemic side effects , and poor adherence to therapy .
	manualset3
165126	2	412418	7	NULL	NULL	0	NULL	effectiveness	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The safety and effectiveness of systemic and topical medical therapies for ocular disorders are limited due to poor ocular drug uptake , nonspecificity to target tissues , systemic side effects , and poor adherence to therapy .
	manualset3
165127	3	412418	7	NULL	NULL	0	NULL	 systemic medical therapies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The safety and effectiveness of systemic and topical medical therapies for ocular disorders are limited due to poor ocular drug uptake , nonspecificity to target tissues , systemic side effects , and poor adherence to therapy .
	manualset3
165128	4	412418	7	NULL	NULL	0	NULL	topical medical therapies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The safety and effectiveness of systemic and topical medical therapies for ocular disorders are limited due to poor ocular drug uptake , nonspecificity to target tissues , systemic side effects , and poor adherence to therapy .
	manualset3
165129	5	412418	7	NULL	NULL	0	NULL	ocular disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The safety and effectiveness of systemic and topical medical therapies for ocular disorders are limited due to poor ocular drug uptake , nonspecificity to target tissues , systemic side effects , and poor adherence to therapy .
	manualset3
165130	6	412418	7	NULL	NULL	0	NULL	poor ocular drug uptake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The safety and effectiveness of systemic and topical medical therapies for ocular disorders are limited due to poor ocular drug uptake , nonspecificity to target tissues , systemic side effects , and poor adherence to therapy .
	manualset3
165131	7	412418	7	NULL	NULL	0	NULL	 target tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The safety and effectiveness of systemic and topical medical therapies for ocular disorders are limited due to poor ocular drug uptake , nonspecificity to target tissues , systemic side effects , and poor adherence to therapy .
	manualset3
165132	8	412418	7	NULL	NULL	0	NULL	systemic side effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The safety and effectiveness of systemic and topical medical therapies for ocular disorders are limited due to poor ocular drug uptake , nonspecificity to target tissues , systemic side effects , and poor adherence to therapy .
	manualset3
165133	9	412418	7	NULL	NULL	0	NULL	poor adherence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The safety and effectiveness of systemic and topical medical therapies for ocular disorders are limited due to poor ocular drug uptake , nonspecificity to target tissues , systemic side effects , and poor adherence to therapy .
	manualset3
165134	10	412418	7	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The safety and effectiveness of systemic and topical medical therapies for ocular disorders are limited due to poor ocular drug uptake , nonspecificity to target tissues , systemic side effects , and poor adherence to therapy .
	manualset3
165135	1	412419	7	NULL	NULL	0	NULL	saline control group 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The saline control group performed DRL responding in an efficient manner with a major index for the peak time of the IRT curve , which was fairly localized within the 10-sec bin throughout the test phase .
	manualset3
165136	2	412419	7	NULL	NULL	0	NULL	DRL	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The saline control group performed DRL responding in an efficient manner with a major index for the peak time of the IRT curve , which was fairly localized within the 10-sec bin throughout the test phase .
	manualset3
165137	3	412419	7	NULL	NULL	0	NULL	efficient manner	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The saline control group performed DRL responding in an efficient manner with a major index for the peak time of the IRT curve , which was fairly localized within the 10-sec bin throughout the test phase .
	manualset3
165138	4	412419	7	NULL	NULL	0	NULL	index	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The saline control group performed DRL responding in an efficient manner with a major index for the peak time of the IRT curve , which was fairly localized within the 10-sec bin throughout the test phase .
	manualset3
165139	5	412419	7	NULL	NULL	0	NULL	peak time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The saline control group performed DRL responding in an efficient manner with a major index for the peak time of the IRT curve , which was fairly localized within the 10-sec bin throughout the test phase .
	manualset3
165140	6	412419	7	NULL	NULL	0	NULL	IRT curve	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The saline control group performed DRL responding in an efficient manner with a major index for the peak time of the IRT curve , which was fairly localized within the 10-sec bin throughout the test phase .
	manualset3
165141	7	412419	7	NULL	NULL	0	NULL	10-sec bin	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The saline control group performed DRL responding in an efficient manner with a major index for the peak time of the IRT curve , which was fairly localized within the 10-sec bin throughout the test phase .
	manualset3
165142	8	412419	7	NULL	NULL	0	NULL	test phase	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The saline control group performed DRL responding in an efficient manner with a major index for the peak time of the IRT curve , which was fairly localized within the 10-sec bin throughout the test phase .
	manualset3
165143	1	412420	7	NULL	NULL	0	NULL	salt	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The salt is stabilized by an extensive network of N-HCl and C-HCl hydrogen bonds , where hydrogen-bonded anion chains and characteristic cation-anion motifs are present .
	manualset3
165144	2	412420	7	NULL	NULL	0	NULL	extensive network	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The salt is stabilized by an extensive network of N-HCl and C-HCl hydrogen bonds , where hydrogen-bonded anion chains and characteristic cation-anion motifs are present .
	manualset3
165145	3	412420	7	NULL	NULL	0	NULL	N-HCl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The salt is stabilized by an extensive network of N-HCl and C-HCl hydrogen bonds , where hydrogen-bonded anion chains and characteristic cation-anion motifs are present .
	manualset3
165146	4	412420	7	NULL	NULL	0	NULL	C-HCl hydrogen bonds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The salt is stabilized by an extensive network of N-HCl and C-HCl hydrogen bonds , where hydrogen-bonded anion chains and characteristic cation-anion motifs are present .
	manualset3
165147	5	412420	7	NULL	NULL	0	NULL	hydrogen-bonded anion chains 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The salt is stabilized by an extensive network of N-HCl and C-HCl hydrogen bonds , where hydrogen-bonded anion chains and characteristic cation-anion motifs are present .
	manualset3
165148	6	412420	7	NULL	NULL	0	NULL	cation-anion motifs 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The salt is stabilized by an extensive network of N-HCl and C-HCl hydrogen bonds , where hydrogen-bonded anion chains and characteristic cation-anion motifs are present .
	manualset3
165149	1	412421	7	NULL	NULL	0	NULL	DNA samples	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The same DNA samples were also analyzed using 32P-postlabeling techniques ( thin-layer chromatography or high-performance liquid chromatography ) to confirm the presence of DNA adducts and estimate their levels .
	manualset3
165150	2	412421	7	NULL	NULL	0	NULL	32P-postlabeling techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The same DNA samples were also analyzed using 32P-postlabeling techniques ( thin-layer chromatography or high-performance liquid chromatography ) to confirm the presence of DNA adducts and estimate their levels .
	manualset3
165151	3	412421	7	NULL	NULL	0	NULL	thin-layer chromatography 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The same DNA samples were also analyzed using 32P-postlabeling techniques ( thin-layer chromatography or high-performance liquid chromatography ) to confirm the presence of DNA adducts and estimate their levels .
	manualset3
165152	4	412421	7	NULL	NULL	0	NULL	 high-performance liquid chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The same DNA samples were also analyzed using 32P-postlabeling techniques ( thin-layer chromatography or high-performance liquid chromatography ) to confirm the presence of DNA adducts and estimate their levels .
	manualset3
165153	5	412421	7	NULL	NULL	0	NULL	DNA adducts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The same DNA samples were also analyzed using 32P-postlabeling techniques ( thin-layer chromatography or high-performance liquid chromatography ) to confirm the presence of DNA adducts and estimate their levels .
	manualset3
165154	6	412421	7	NULL	NULL	0	NULL	levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The same DNA samples were also analyzed using 32P-postlabeling techniques ( thin-layer chromatography or high-performance liquid chromatography ) to confirm the presence of DNA adducts and estimate their levels .
	manualset3
172019	7	412421	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The same DNA samples were also analyzed using 32P-postlabeling techniques ( thin-layer chromatography or high-performance liquid chromatography ) to confirm the presence of DNA adducts and estimate their levels .
	manualset3
165155	1	412422	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our data we propose that thymopentin has stress-protective activity .
	manualset3
165156	2	412422	7	NULL	NULL	0	NULL	thymopentin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our data we propose that thymopentin has stress-protective activity .
	manualset3
165157	3	412422	7	NULL	NULL	0	NULL	stress-protective activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our data we propose that thymopentin has stress-protective activity .
	manualset3
165158	1	412423	7	NULL	NULL	0	NULL	dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The same dose of t-PA infused over 60 , 30 and 15 minutes produced 87 % , 88 % and 96 % thrombolysis , respectively ( p less than 0.01 ) .
	manualset3
165159	2	412423	7	NULL	NULL	0	NULL	t-PA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The same dose of t-PA infused over 60 , 30 and 15 minutes produced 87 % , 88 % and 96 % thrombolysis , respectively ( p less than 0.01 ) .
	manualset3
165160	3	412423	7	NULL	NULL	0	NULL	60 minutes	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The same dose of t-PA infused over 60 , 30 and 15 minutes produced 87 % , 88 % and 96 % thrombolysis , respectively ( p less than 0.01 ) .
	manualset3
165161	4	412423	7	NULL	NULL	0	NULL	30 minutes	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The same dose of t-PA infused over 60 , 30 and 15 minutes produced 87 % , 88 % and 96 % thrombolysis , respectively ( p less than 0.01 ) .
	manualset3
165162	5	412423	7	NULL	NULL	0	NULL	15 minutes	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The same dose of t-PA infused over 60 , 30 and 15 minutes produced 87 % , 88 % and 96 % thrombolysis , respectively ( p less than 0.01 ) .
	manualset3
165163	6	412423	7	NULL	NULL	0	NULL	87 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The same dose of t-PA infused over 60 , 30 and 15 minutes produced 87 % , 88 % and 96 % thrombolysis , respectively ( p less than 0.01 ) .
	manualset3
165164	7	412423	7	NULL	NULL	0	NULL	88 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The same dose of t-PA infused over 60 , 30 and 15 minutes produced 87 % , 88 % and 96 % thrombolysis , respectively ( p less than 0.01 ) .
	manualset3
165165	8	412423	7	NULL	NULL	0	NULL	96 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The same dose of t-PA infused over 60 , 30 and 15 minutes produced 87 % , 88 % and 96 % thrombolysis , respectively ( p less than 0.01 ) .
	manualset3
165166	9	412423	7	NULL	NULL	0	NULL	thrombolysis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The same dose of t-PA infused over 60 , 30 and 15 minutes produced 87 % , 88 % and 96 % thrombolysis , respectively ( p less than 0.01 ) .
	manualset3
165167	10	412423	7	NULL	NULL	0	NULL	p less than 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The same dose of t-PA infused over 60 , 30 and 15 minutes produced 87 % , 88 % and 96 % thrombolysis , respectively ( p less than 0.01 ) .
	manualset3
165168	1	412424	7	NULL	NULL	NULL	NULL	 fractions	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The same fractions analyzed by GC-MS , and a separate set of polar fractions , were evaluated against two life cycle stages ( epimastigote and trypomastigote forms ) of the protozoan Trypanosoma cruzi and against phytopatogenic fungi Cladosporium cladosporiodes and C. sphaerospermum .
	manualset3
165169	2	412424	7	NULL	NULL	0	NULL	GC-MS	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The same fractions analyzed by GC-MS , and a separate set of polar fractions , were evaluated against two life cycle stages ( epimastigote and trypomastigote forms ) of the protozoan Trypanosoma cruzi and against phytopatogenic fungi Cladosporium cladosporiodes and C. sphaerospermum .
	manualset3
165170	3	412424	7	NULL	NULL	0	NULL	 polar fractions	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The same fractions analyzed by GC-MS , and a separate set of polar fractions , were evaluated against two life cycle stages ( epimastigote and trypomastigote forms ) of the protozoan Trypanosoma cruzi and against phytopatogenic fungi Cladosporium cladosporiodes and C. sphaerospermum .
	manualset3
165171	4	412424	7	NULL	NULL	NULL	NULL	two life cycle stages	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The same fractions analyzed by GC-MS , and a separate set of polar fractions , were evaluated against two life cycle stages ( epimastigote and trypomastigote forms ) of the protozoan Trypanosoma cruzi and against phytopatogenic fungi Cladosporium cladosporiodes and C. sphaerospermum .
	manualset3
165172	5	412424	7	NULL	NULL	0	NULL	epimastigote forms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The same fractions analyzed by GC-MS , and a separate set of polar fractions , were evaluated against two life cycle stages ( epimastigote and trypomastigote forms ) of the protozoan Trypanosoma cruzi and against phytopatogenic fungi Cladosporium cladosporiodes and C. sphaerospermum .
	manualset3
165173	6	412424	7	NULL	NULL	0	NULL	trypomastigote forms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The same fractions analyzed by GC-MS , and a separate set of polar fractions , were evaluated against two life cycle stages ( epimastigote and trypomastigote forms ) of the protozoan Trypanosoma cruzi and against phytopatogenic fungi Cladosporium cladosporiodes and C. sphaerospermum .
	manualset3
165174	7	412424	7	NULL	NULL	0	NULL	protozoan Trypanosoma cruzi	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The same fractions analyzed by GC-MS , and a separate set of polar fractions , were evaluated against two life cycle stages ( epimastigote and trypomastigote forms ) of the protozoan Trypanosoma cruzi and against phytopatogenic fungi Cladosporium cladosporiodes and C. sphaerospermum .
	manualset3
165175	8	412424	7	NULL	NULL	0	NULL	phytopatogenic fungi Cladosporium cladosporiodes 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The same fractions analyzed by GC-MS , and a separate set of polar fractions , were evaluated against two life cycle stages ( epimastigote and trypomastigote forms ) of the protozoan Trypanosoma cruzi and against phytopatogenic fungi Cladosporium cladosporiodes and C. sphaerospermum .
	manualset3
165176	9	412424	7	NULL	NULL	0	NULL	C. sphaerospermum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The same fractions analyzed by GC-MS , and a separate set of polar fractions , were evaluated against two life cycle stages ( epimastigote and trypomastigote forms ) of the protozoan Trypanosoma cruzi and against phytopatogenic fungi Cladosporium cladosporiodes and C. sphaerospermum .
	manualset3
165177	1	412425	7	NULL	NULL	0	NULL	 procedure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The same procedure is used to optimize a levitator consisting of a curved reflector and a concave-faced transducer .
	manualset3
165178	2	412425	7	NULL	NULL	NULL	NULL	levitator	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The same procedure is used to optimize a levitator consisting of a curved reflector and a concave-faced transducer .
	manualset3
165179	3	412425	7	NULL	NULL	0	NULL	curved reflector	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The same procedure is used to optimize a levitator consisting of a curved reflector and a concave-faced transducer .
	manualset3
165180	4	412425	7	NULL	NULL	0	NULL	concave-faced transducer	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The same procedure is used to optimize a levitator consisting of a curved reflector and a concave-faced transducer .
	manualset3
165181	1	412426	7	NULL	NULL	0	NULL	yields	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The same yields were obtained in phosphate buffer at 3 degrees and 22 degrees as well as in growth medium at 37 degrees , and the yields were not altered by the polA1 mutation .
	manualset3
165182	2	412426	7	NULL	NULL	0	NULL	phosphate buffer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The same yields were obtained in phosphate buffer at 3 degrees and 22 degrees as well as in growth medium at 37 degrees , and the yields were not altered by the polA1 mutation .
	manualset3
165183	3	412426	7	NULL	NULL	0	NULL	3 degrees	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The same yields were obtained in phosphate buffer at 3 degrees and 22 degrees as well as in growth medium at 37 degrees , and the yields were not altered by the polA1 mutation .
	manualset3
165184	4	412426	7	NULL	NULL	0	NULL	22 degrees	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The same yields were obtained in phosphate buffer at 3 degrees and 22 degrees as well as in growth medium at 37 degrees , and the yields were not altered by the polA1 mutation .
	manualset3
165185	5	412426	7	NULL	NULL	0	NULL	 growth medium	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The same yields were obtained in phosphate buffer at 3 degrees and 22 degrees as well as in growth medium at 37 degrees , and the yields were not altered by the polA1 mutation .
	manualset3
165186	6	412426	7	NULL	NULL	0	NULL	37 degrees	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The same yields were obtained in phosphate buffer at 3 degrees and 22 degrees as well as in growth medium at 37 degrees , and the yields were not altered by the polA1 mutation .
	manualset3
165187	7	412426	7	NULL	NULL	0	NULL	yields	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The same yields were obtained in phosphate buffer at 3 degrees and 22 degrees as well as in growth medium at 37 degrees , and the yields were not altered by the polA1 mutation .
	manualset3
165188	8	412426	7	NULL	NULL	0	NULL	polA1 mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The same yields were obtained in phosphate buffer at 3 degrees and 22 degrees as well as in growth medium at 37 degrees , and the yields were not altered by the polA1 mutation .
	manualset3
165189	1	412427	7	NULL	NULL	0	NULL	sample capacity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample capacity , column efficiency ( and its variation with flow ) of a superficially porous unbonded silica phase ( Halo ) was investigated using hydrophilic interaction chromatography ( HILIC ) , particularly for separation of basic compounds .
	manualset3
165190	2	412427	7	NULL	NULL	0	NULL	column efficiency	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample capacity , column efficiency ( and its variation with flow ) of a superficially porous unbonded silica phase ( Halo ) was investigated using hydrophilic interaction chromatography ( HILIC ) , particularly for separation of basic compounds .
	manualset3
165191	3	412427	7	NULL	NULL	0	NULL	variation with flow 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample capacity , column efficiency ( and its variation with flow ) of a superficially porous unbonded silica phase ( Halo ) was investigated using hydrophilic interaction chromatography ( HILIC ) , particularly for separation of basic compounds .
	manualset3
165192	4	412427	7	NULL	NULL	0	NULL	superficially porous unbonded silica phase ( Halo )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample capacity , column efficiency ( and its variation with flow ) of a superficially porous unbonded silica phase ( Halo ) was investigated using hydrophilic interaction chromatography ( HILIC ) , particularly for separation of basic compounds .
	manualset3
165193	5	412427	7	NULL	NULL	0	NULL	hydrophilic interaction chromatography ( HILIC )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample capacity , column efficiency ( and its variation with flow ) of a superficially porous unbonded silica phase ( Halo ) was investigated using hydrophilic interaction chromatography ( HILIC ) , particularly for separation of basic compounds .
	manualset3
165194	6	412427	7	NULL	NULL	0	NULL	separation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample capacity , column efficiency ( and its variation with flow ) of a superficially porous unbonded silica phase ( Halo ) was investigated using hydrophilic interaction chromatography ( HILIC ) , particularly for separation of basic compounds .
	manualset3
165195	7	412427	7	NULL	NULL	0	NULL	basic compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample capacity , column efficiency ( and its variation with flow ) of a superficially porous unbonded silica phase ( Halo ) was investigated using hydrophilic interaction chromatography ( HILIC ) , particularly for separation of basic compounds .
	manualset3
165196	1	412428	7	NULL	NULL	0	NULL	sample 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample consisted of 57 men and 3 women aged 34 to 69 years ( mean + / - SD : 46.8 + / - 6.9 ) .
	manualset3
165197	2	412428	7	NULL	NULL	0	NULL	57 men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample consisted of 57 men and 3 women aged 34 to 69 years ( mean + / - SD : 46.8 + / - 6.9 ) .
	manualset3
165198	3	412428	7	NULL	NULL	0	NULL	3 women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample consisted of 57 men and 3 women aged 34 to 69 years ( mean + / - SD : 46.8 + / - 6.9 ) .
	manualset3
165199	4	412428	7	NULL	NULL	0	NULL	34 to 69 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample consisted of 57 men and 3 women aged 34 to 69 years ( mean + / - SD : 46.8 + / - 6.9 ) .
	manualset3
165200	5	412428	7	NULL	NULL	0	NULL	mean + / - SD : 46.8 + / - 6.9	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample consisted of 57 men and 3 women aged 34 to 69 years ( mean + / - SD : 46.8 + / - 6.9 ) .
	manualset3
165201	1	412429	7	NULL	NULL	0	NULL	sample	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample consisted of two similar-sized anatids , Aix sponsa ( n = 7 ) and Oxyura jamaicensis ( n = 5 ) .
	manualset3
165202	2	412429	7	NULL	NULL	0	NULL	two similar-sized anatids	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample consisted of two similar-sized anatids , Aix sponsa ( n = 7 ) and Oxyura jamaicensis ( n = 5 ) .
	manualset3
165203	3	412429	7	NULL	NULL	0	NULL	Aix sponsa	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample consisted of two similar-sized anatids , Aix sponsa ( n = 7 ) and Oxyura jamaicensis ( n = 5 ) .
	manualset3
165204	4	412429	7	NULL	NULL	0	NULL	n = 7	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample consisted of two similar-sized anatids , Aix sponsa ( n = 7 ) and Oxyura jamaicensis ( n = 5 ) .
	manualset3
165205	5	412429	7	NULL	NULL	0	NULL	Oxyura jamaicensis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample consisted of two similar-sized anatids , Aix sponsa ( n = 7 ) and Oxyura jamaicensis ( n = 5 ) .
	manualset3
165206	6	412429	7	NULL	NULL	0	NULL	 n = 5	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample consisted of two similar-sized anatids , Aix sponsa ( n = 7 ) and Oxyura jamaicensis ( n = 5 ) .
	manualset3
165207	1	412430	7	NULL	NULL	0	NULL	sample	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample consisted of women in the screening program who received an abnormal cervical screening result ( N = 1.738 ) .
	manualset3
165208	2	412430	7	NULL	NULL	0	NULL	 women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample consisted of women in the screening program who received an abnormal cervical screening result ( N = 1.738 ) .
	manualset3
165209	3	412430	7	NULL	NULL	0	NULL	screening program	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample consisted of women in the screening program who received an abnormal cervical screening result ( N = 1.738 ) .
	manualset3
165210	4	412430	7	NULL	NULL	0	NULL	abnormal cervical screening result	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample consisted of women in the screening program who received an abnormal cervical screening result ( N = 1.738 ) .
	manualset3
165211	5	412430	7	NULL	NULL	0	NULL	N = 1.738	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample consisted of women in the screening program who received an abnormal cervical screening result ( N = 1.738 ) .
	manualset3
165229	1	412431	7	NULL	NULL	0	NULL	field study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our field study , acetaldehyde ( 19.5 + / -10.6 ppb ) and formaldehyde ( 19.3 + / -10.1 ppb ) were found to be the two most abundant species followed by propionaldehyde ( 19.0 + / -23.2 ppb ) , acetone ( 15.9 + / -15.2 ppb ) and butyraldehyde ( 13.0 + / -19.8 ppb ) .
	manualset3
165230	2	412431	7	NULL	NULL	0	NULL	 acetaldehyde	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our field study , acetaldehyde ( 19.5 + / -10.6 ppb ) and formaldehyde ( 19.3 + / -10.1 ppb ) were found to be the two most abundant species followed by propionaldehyde ( 19.0 + / -23.2 ppb ) , acetone ( 15.9 + / -15.2 ppb ) and butyraldehyde ( 13.0 + / -19.8 ppb ) .
	manualset3
165231	3	412431	7	NULL	NULL	0	NULL	19.5 + / -10.6 ppb	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our field study , acetaldehyde ( 19.5 + / -10.6 ppb ) and formaldehyde ( 19.3 + / -10.1 ppb ) were found to be the two most abundant species followed by propionaldehyde ( 19.0 + / -23.2 ppb ) , acetone ( 15.9 + / -15.2 ppb ) and butyraldehyde ( 13.0 + / -19.8 ppb ) .
	manualset3
165232	4	412431	7	NULL	NULL	0	NULL	 formaldehyde 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our field study , acetaldehyde ( 19.5 + / -10.6 ppb ) and formaldehyde ( 19.3 + / -10.1 ppb ) were found to be the two most abundant species followed by propionaldehyde ( 19.0 + / -23.2 ppb ) , acetone ( 15.9 + / -15.2 ppb ) and butyraldehyde ( 13.0 + / -19.8 ppb ) .
	manualset3
165233	5	412431	7	NULL	NULL	0	NULL	19.3 + / -10.1 ppb	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our field study , acetaldehyde ( 19.5 + / -10.6 ppb ) and formaldehyde ( 19.3 + / -10.1 ppb ) were found to be the two most abundant species followed by propionaldehyde ( 19.0 + / -23.2 ppb ) , acetone ( 15.9 + / -15.2 ppb ) and butyraldehyde ( 13.0 + / -19.8 ppb ) .
	manualset3
165234	6	412431	7	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our field study , acetaldehyde ( 19.5 + / -10.6 ppb ) and formaldehyde ( 19.3 + / -10.1 ppb ) were found to be the two most abundant species followed by propionaldehyde ( 19.0 + / -23.2 ppb ) , acetone ( 15.9 + / -15.2 ppb ) and butyraldehyde ( 13.0 + / -19.8 ppb ) .
	manualset3
165235	7	412431	7	NULL	NULL	0	NULL	abundant species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our field study , acetaldehyde ( 19.5 + / -10.6 ppb ) and formaldehyde ( 19.3 + / -10.1 ppb ) were found to be the two most abundant species followed by propionaldehyde ( 19.0 + / -23.2 ppb ) , acetone ( 15.9 + / -15.2 ppb ) and butyraldehyde ( 13.0 + / -19.8 ppb ) .
	manualset3
165236	8	412431	7	NULL	NULL	0	NULL	propionaldehyde	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our field study , acetaldehyde ( 19.5 + / -10.6 ppb ) and formaldehyde ( 19.3 + / -10.1 ppb ) were found to be the two most abundant species followed by propionaldehyde ( 19.0 + / -23.2 ppb ) , acetone ( 15.9 + / -15.2 ppb ) and butyraldehyde ( 13.0 + / -19.8 ppb ) .
	manualset3
165237	9	412431	7	NULL	NULL	0	NULL	19.0 + / -23.2 ppb	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our field study , acetaldehyde ( 19.5 + / -10.6 ppb ) and formaldehyde ( 19.3 + / -10.1 ppb ) were found to be the two most abundant species followed by propionaldehyde ( 19.0 + / -23.2 ppb ) , acetone ( 15.9 + / -15.2 ppb ) and butyraldehyde ( 13.0 + / -19.8 ppb ) .
	manualset3
165238	10	412431	7	NULL	NULL	0	NULL	acetone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our field study , acetaldehyde ( 19.5 + / -10.6 ppb ) and formaldehyde ( 19.3 + / -10.1 ppb ) were found to be the two most abundant species followed by propionaldehyde ( 19.0 + / -23.2 ppb ) , acetone ( 15.9 + / -15.2 ppb ) and butyraldehyde ( 13.0 + / -19.8 ppb ) .
	manualset3
165239	11	412431	7	NULL	NULL	0	NULL	15.9 + / -15.2 ppb	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our field study , acetaldehyde ( 19.5 + / -10.6 ppb ) and formaldehyde ( 19.3 + / -10.1 ppb ) were found to be the two most abundant species followed by propionaldehyde ( 19.0 + / -23.2 ppb ) , acetone ( 15.9 + / -15.2 ppb ) and butyraldehyde ( 13.0 + / -19.8 ppb ) .
	manualset3
165240	12	412431	7	NULL	NULL	0	NULL	butyraldehyde	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our field study , acetaldehyde ( 19.5 + / -10.6 ppb ) and formaldehyde ( 19.3 + / -10.1 ppb ) were found to be the two most abundant species followed by propionaldehyde ( 19.0 + / -23.2 ppb ) , acetone ( 15.9 + / -15.2 ppb ) and butyraldehyde ( 13.0 + / -19.8 ppb ) .
	manualset3
165241	13	412431	7	NULL	NULL	0	NULL	13.0 + / -19.8 ppb	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our field study , acetaldehyde ( 19.5 + / -10.6 ppb ) and formaldehyde ( 19.3 + / -10.1 ppb ) were found to be the two most abundant species followed by propionaldehyde ( 19.0 + / -23.2 ppb ) , acetone ( 15.9 + / -15.2 ppb ) and butyraldehyde ( 13.0 + / -19.8 ppb ) .
	manualset3
165242	1	412432	7	NULL	NULL	0	NULL	sample handling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample handling and data processing have been significantly automated , and the protocol has been applied to over 800 in-house lead molecules to date .
	manualset3
165243	2	412432	7	NULL	NULL	0	NULL	data processing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample handling and data processing have been significantly automated , and the protocol has been applied to over 800 in-house lead molecules to date .
	manualset3
165244	3	412432	7	NULL	NULL	0	NULL	protocol 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample handling and data processing have been significantly automated , and the protocol has been applied to over 800 in-house lead molecules to date .
	manualset3
165245	4	412432	7	NULL	NULL	0	NULL	800	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample handling and data processing have been significantly automated , and the protocol has been applied to over 800 in-house lead molecules to date .
	manualset3
165246	5	412432	7	NULL	NULL	0	NULL	in-house lead molecules	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample handling and data processing have been significantly automated , and the protocol has been applied to over 800 in-house lead molecules to date .
	manualset3
165247	6	412432	7	NULL	NULL	0	NULL	date 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample handling and data processing have been significantly automated , and the protocol has been applied to over 800 in-house lead molecules to date .
	manualset3
165248	1	412433	7	NULL	NULL	0	NULL	sample	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample involved 212 men and 212 women , most of whom are overweight and obese .
	manualset3
165249	2	412433	7	NULL	NULL	0	NULL	212 men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample involved 212 men and 212 women , most of whom are overweight and obese .
	manualset3
165250	3	412433	7	NULL	NULL	0	NULL	 212 women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample involved 212 men and 212 women , most of whom are overweight and obese .
	manualset3
165253	1	412434	7	NULL	NULL	0	NULL	sample	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample of 338 persons was drawn from university students and community residents .
	manualset3
165254	2	412434	7	NULL	NULL	0	NULL	338 persons	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample of 338 persons was drawn from university students and community residents .
	manualset3
165255	3	412434	7	NULL	NULL	0	NULL	university students	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample of 338 persons was drawn from university students and community residents .
	manualset3
165256	4	412434	7	NULL	NULL	0	NULL	community residents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The sample of 338 persons was drawn from university students and community residents .
	manualset3
165257	1	412435	7	NULL	NULL	0	NULL	 samples	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The samples ( 10-l aliquot ) were fortified with stable-labeled internal standard ( d18-atrasentan ) and lysed thoroughly prior to protein precipitation .
	manualset3
165258	2	412435	7	NULL	NULL	0	NULL	10-l aliquot 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The samples ( 10-l aliquot ) were fortified with stable-labeled internal standard ( d18-atrasentan ) and lysed thoroughly prior to protein precipitation .
	manualset3
165259	3	412435	7	NULL	NULL	0	NULL	stable-labeled internal standard	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The samples ( 10-l aliquot ) were fortified with stable-labeled internal standard ( d18-atrasentan ) and lysed thoroughly prior to protein precipitation .
	manualset3
165260	4	412435	7	NULL	NULL	0	NULL	d18-atrasentan	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The samples ( 10-l aliquot ) were fortified with stable-labeled internal standard ( d18-atrasentan ) and lysed thoroughly prior to protein precipitation .
	manualset3
165261	5	412435	7	NULL	NULL	0	NULL	protein precipitation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The samples ( 10-l aliquot ) were fortified with stable-labeled internal standard ( d18-atrasentan ) and lysed thoroughly prior to protein precipitation .
	manualset3
165262	1	412436	7	NULL	NULL	0	NULL	sampling site	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The sampling site was divided into two regions for analysis : ( a ) .
	manualset3
165263	2	412436	7	NULL	NULL	0	NULL	 two regions	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The sampling site was divided into two regions for analysis : ( a ) .
	manualset3
165264	3	412436	7	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The sampling site was divided into two regions for analysis : ( a ) .
	manualset3
165265	1	412437	7	NULL	NULL	0	NULL	sarcoglycans	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The sarcoglycans are known as an integral subcomplex of the dystrophin glycoprotein complex , the function of which is best characterized in skeletal muscle in relation to muscular dystrophies .
	manualset3
165266	2	412437	7	NULL	NULL	0	NULL	integral subcomplex	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The sarcoglycans are known as an integral subcomplex of the dystrophin glycoprotein complex , the function of which is best characterized in skeletal muscle in relation to muscular dystrophies .
	manualset3
165267	3	412437	7	NULL	NULL	NULL	NULL	dystrophin glycoprotein complex	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The sarcoglycans are known as an integral subcomplex of the dystrophin glycoprotein complex , the function of which is best characterized in skeletal muscle in relation to muscular dystrophies .
	manualset3
165268	4	412437	7	NULL	NULL	0	NULL	 function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The sarcoglycans are known as an integral subcomplex of the dystrophin glycoprotein complex , the function of which is best characterized in skeletal muscle in relation to muscular dystrophies .
	manualset3
165269	5	412437	7	NULL	NULL	0	NULL	skeletal muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The sarcoglycans are known as an integral subcomplex of the dystrophin glycoprotein complex , the function of which is best characterized in skeletal muscle in relation to muscular dystrophies .
	manualset3
165270	6	412437	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The sarcoglycans are known as an integral subcomplex of the dystrophin glycoprotein complex , the function of which is best characterized in skeletal muscle in relation to muscular dystrophies .
	manualset3
165271	7	412437	7	NULL	NULL	0	NULL	muscular dystrophies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The sarcoglycans are known as an integral subcomplex of the dystrophin glycoprotein complex , the function of which is best characterized in skeletal muscle in relation to muscular dystrophies .
	manualset3
165272	1	412438	7	NULL	NULL	0	NULL	saturation functions	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The saturation functions by citrulline and aspartate are hyperbolic ; with MgATP as the variable substrate a sigmoid character , dependent on the concentration of citrulline , aspartate , argininosuccinate and arginine , was observed .
	manualset3
165273	2	412438	7	NULL	NULL	0	NULL	citrulline 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The saturation functions by citrulline and aspartate are hyperbolic ; with MgATP as the variable substrate a sigmoid character , dependent on the concentration of citrulline , aspartate , argininosuccinate and arginine , was observed .
	manualset3
165274	3	412438	7	NULL	NULL	NULL	NULL	aspartate	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The saturation functions by citrulline and aspartate are hyperbolic ; with MgATP as the variable substrate a sigmoid character , dependent on the concentration of citrulline , aspartate , argininosuccinate and arginine , was observed .
	manualset3
165275	4	412438	7	NULL	NULL	0	NULL	MgATP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The saturation functions by citrulline and aspartate are hyperbolic ; with MgATP as the variable substrate a sigmoid character , dependent on the concentration of citrulline , aspartate , argininosuccinate and arginine , was observed .
	manualset3
165276	5	412438	7	NULL	NULL	0	NULL	variable substrate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The saturation functions by citrulline and aspartate are hyperbolic ; with MgATP as the variable substrate a sigmoid character , dependent on the concentration of citrulline , aspartate , argininosuccinate and arginine , was observed .
	manualset3
165277	6	412438	7	NULL	NULL	0	NULL	sigmoid character	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The saturation functions by citrulline and aspartate are hyperbolic ; with MgATP as the variable substrate a sigmoid character , dependent on the concentration of citrulline , aspartate , argininosuccinate and arginine , was observed .
	manualset3
165278	7	412438	7	NULL	NULL	0	NULL	concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The saturation functions by citrulline and aspartate are hyperbolic ; with MgATP as the variable substrate a sigmoid character , dependent on the concentration of citrulline , aspartate , argininosuccinate and arginine , was observed .
	manualset3
165279	8	412438	7	NULL	NULL	0	NULL	citrulline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The saturation functions by citrulline and aspartate are hyperbolic ; with MgATP as the variable substrate a sigmoid character , dependent on the concentration of citrulline , aspartate , argininosuccinate and arginine , was observed .
	manualset3
165280	9	412438	7	NULL	NULL	0	NULL	aspartate	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The saturation functions by citrulline and aspartate are hyperbolic ; with MgATP as the variable substrate a sigmoid character , dependent on the concentration of citrulline , aspartate , argininosuccinate and arginine , was observed .
	manualset3
165281	10	412438	7	NULL	NULL	0	NULL	argininosuccinate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The saturation functions by citrulline and aspartate are hyperbolic ; with MgATP as the variable substrate a sigmoid character , dependent on the concentration of citrulline , aspartate , argininosuccinate and arginine , was observed .
	manualset3
165282	11	412438	7	NULL	NULL	0	NULL	arginine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The saturation functions by citrulline and aspartate are hyperbolic ; with MgATP as the variable substrate a sigmoid character , dependent on the concentration of citrulline , aspartate , argininosuccinate and arginine , was observed .
	manualset3
165283	1	412439	7	NULL	NULL	0	NULL	scale items	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The scale items reflect the four categories of the induced definition of hope and comprise the inductively developed ` Hopefulness Scale for Adolescents ' .
	manualset3
165284	2	412439	7	NULL	NULL	0	NULL	 four categories	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The scale items reflect the four categories of the induced definition of hope and comprise the inductively developed ` Hopefulness Scale for Adolescents ' .
	manualset3
165285	3	412439	7	NULL	NULL	0	NULL	definition of hope	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The scale items reflect the four categories of the induced definition of hope and comprise the inductively developed ` Hopefulness Scale for Adolescents ' .
	manualset3
165286	4	412439	7	NULL	NULL	0	NULL	Hopefulness Scale for Adolescents	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The scale items reflect the four categories of the induced definition of hope and comprise the inductively developed ` Hopefulness Scale for Adolescents ' .
	manualset3
165287	1	412440	7	NULL	NULL	NULL	NULL	opinion	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	According to our opinion , ethical questions should not be regulated by law and the legal system should not interfere in the relationship patient - physician .
	manualset3
165288	2	412440	7	NULL	NULL	NULL	NULL	ethical questions 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	According to our opinion , ethical questions should not be regulated by law and the legal system should not interfere in the relationship patient - physician .
	manualset3
165289	3	412440	7	NULL	NULL	0	NULL	 law	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our opinion , ethical questions should not be regulated by law and the legal system should not interfere in the relationship patient - physician .
	manualset3
165290	4	412440	7	NULL	NULL	0	NULL	legal system	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our opinion , ethical questions should not be regulated by law and the legal system should not interfere in the relationship patient - physician .
	manualset3
165291	5	412440	7	NULL	NULL	0	NULL	 relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our opinion , ethical questions should not be regulated by law and the legal system should not interfere in the relationship patient - physician .
	manualset3
165292	6	412440	7	NULL	NULL	0	NULL	patient - physician	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our opinion , ethical questions should not be regulated by law and the legal system should not interfere in the relationship patient - physician .
	manualset3
165293	1	412441	7	NULL	NULL	0	NULL	scalp lipid content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The scalp lipid content remained unaltered in 11 patients with an initial lipid value over 220 micrograms/cm2 but increased in those with lower initial values .
	manualset3
165294	2	412441	7	NULL	NULL	0	NULL	11 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The scalp lipid content remained unaltered in 11 patients with an initial lipid value over 220 micrograms/cm2 but increased in those with lower initial values .
	manualset3
165295	3	412441	7	NULL	NULL	0	NULL	 lipid value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The scalp lipid content remained unaltered in 11 patients with an initial lipid value over 220 micrograms/cm2 but increased in those with lower initial values .
	manualset3
165296	4	412441	7	NULL	NULL	0	NULL	220 micrograms/cm2 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The scalp lipid content remained unaltered in 11 patients with an initial lipid value over 220 micrograms/cm2 but increased in those with lower initial values .
	manualset3
165297	5	412441	7	NULL	NULL	0	NULL	lower initial values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The scalp lipid content remained unaltered in 11 patients with an initial lipid value over 220 micrograms/cm2 but increased in those with lower initial values .
	manualset3
165298	1	412442	7	NULL	NULL	0	NULL	school 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The school psychologist and mild retardation .
	manualset3
165299	2	412442	7	NULL	NULL	0	NULL	psychologist	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The school psychologist and mild retardation .
	manualset3
165300	3	412442	7	NULL	NULL	0	NULL	mild retardation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The school psychologist and mild retardation .
	manualset3
165301	1	412443	7	NULL	NULL	0	NULL	science	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The science of USP 1 and 2 dissolution : present challenges and future relevance .
	manualset3
165302	2	412443	7	NULL	NULL	0	NULL	USP 1 dissolution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The science of USP 1 and 2 dissolution : present challenges and future relevance .
	manualset3
165303	3	412443	7	NULL	NULL	0	NULL	USP 2 dissolution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The science of USP 1 and 2 dissolution : present challenges and future relevance .
	manualset3
165304	4	412443	7	NULL	NULL	0	NULL	challenges	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The science of USP 1 and 2 dissolution : present challenges and future relevance .
	manualset3
173642	5	412443	7	NULL	NULL	0	NULL	relevance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The science of USP 1 and 2 dissolution : present challenges and future relevance .
	manualset3
165305	1	412444	7	NULL	NULL	0	NULL	scientific basis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The scientific basis of gene therapy is introduced and then the current state of research is discussed in relation to the eye and ocular tissues .
	manualset3
165306	2	412444	7	NULL	NULL	0	NULL	gene therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The scientific basis of gene therapy is introduced and then the current state of research is discussed in relation to the eye and ocular tissues .
	manualset3
165307	3	412444	7	NULL	NULL	0	NULL	current state	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The scientific basis of gene therapy is introduced and then the current state of research is discussed in relation to the eye and ocular tissues .
	manualset3
165308	4	412444	7	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The scientific basis of gene therapy is introduced and then the current state of research is discussed in relation to the eye and ocular tissues .
	manualset3
165309	5	412444	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The scientific basis of gene therapy is introduced and then the current state of research is discussed in relation to the eye and ocular tissues .
	manualset3
165310	6	412444	7	NULL	NULL	0	NULL	eye tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The scientific basis of gene therapy is introduced and then the current state of research is discussed in relation to the eye and ocular tissues .
	manualset3
165311	7	412444	7	NULL	NULL	0	NULL	ocular tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The scientific basis of gene therapy is introduced and then the current state of research is discussed in relation to the eye and ocular tissues .
	manualset3
165312	1	412445	7	NULL	NULL	NULL	NULL	scrambled patterns 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The scrambled patterns of the alphaTP gene in the three species are similar but show significant differences .
	manualset3
165313	2	412445	7	NULL	NULL	0	NULL	alphaTP gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The scrambled patterns of the alphaTP gene in the three species are similar but show significant differences .
	manualset3
165314	3	412445	7	NULL	NULL	0	NULL	three species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The scrambled patterns of the alphaTP gene in the three species are similar but show significant differences .
	manualset3
165316	1	412446	7	NULL	NULL	0	NULL	screening	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The screening also provides the Department with better photographic services in general .
	manualset3
165317	2	412446	7	NULL	NULL	0	NULL	Department	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The screening also provides the Department with better photographic services in general .
	manualset3
165318	3	412446	7	NULL	NULL	0	NULL	photographic services	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The screening also provides the Department with better photographic services in general .
	manualset3
165319	1	412447	7	NULL	NULL	0	NULL	 screening extension	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The screening extension increased from 1996 , reaching an overall 68.7 % coverage in 2004 .
	manualset3
165320	2	412447	7	NULL	NULL	0	NULL	1996	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The screening extension increased from 1996 , reaching an overall 68.7 % coverage in 2004 .
	manualset3
165321	3	412447	7	NULL	NULL	0	NULL	68.7 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The screening extension increased from 1996 , reaching an overall 68.7 % coverage in 2004 .
	manualset3
165322	4	412447	7	NULL	NULL	0	NULL	2004	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The screening extension increased from 1996 , reaching an overall 68.7 % coverage in 2004 .
	manualset3
165323	1	412448	7	NULL	NULL	0	NULL	search	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for drug leads targeted to the beta-secretase : an example of the roles of computer assisted approaches in drug discovery .
	manualset3
165324	2	412448	7	NULL	NULL	NULL	NULL	drug leads	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The search for drug leads targeted to the beta-secretase : an example of the roles of computer assisted approaches in drug discovery .
	manualset3
165325	3	412448	7	NULL	NULL	0	NULL	beta-secretase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for drug leads targeted to the beta-secretase : an example of the roles of computer assisted approaches in drug discovery .
	manualset3
165326	4	412448	7	NULL	NULL	NULL	NULL	example	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The search for drug leads targeted to the beta-secretase : an example of the roles of computer assisted approaches in drug discovery .
	manualset3
165327	5	412448	7	NULL	NULL	0	NULL	roles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for drug leads targeted to the beta-secretase : an example of the roles of computer assisted approaches in drug discovery .
	manualset3
165328	6	412448	7	NULL	NULL	0	NULL	computer assisted approaches	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for drug leads targeted to the beta-secretase : an example of the roles of computer assisted approaches in drug discovery .
	manualset3
165329	7	412448	7	NULL	NULL	0	NULL	 drug discovery	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for drug leads targeted to the beta-secretase : an example of the roles of computer assisted approaches in drug discovery .
	manualset3
165330	1	412449	7	NULL	NULL	0	NULL	 search	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for functional foods or functional food ingredients , i.e. foods or food ingredients that can enhance health , is beyond any doubt one of the leading trends in today 's food industry .
	manualset3
165331	2	412449	7	NULL	NULL	0	NULL	functional foods	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for functional foods or functional food ingredients , i.e. foods or food ingredients that can enhance health , is beyond any doubt one of the leading trends in today 's food industry .
	manualset3
165332	3	412449	7	NULL	NULL	0	NULL	functional food ingredients	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for functional foods or functional food ingredients , i.e. foods or food ingredients that can enhance health , is beyond any doubt one of the leading trends in today 's food industry .
	manualset3
165333	4	412449	7	NULL	NULL	0	NULL	 foods	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for functional foods or functional food ingredients , i.e. foods or food ingredients that can enhance health , is beyond any doubt one of the leading trends in today 's food industry .
	manualset3
165334	5	412449	7	NULL	NULL	0	NULL	food ingredients	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for functional foods or functional food ingredients , i.e. foods or food ingredients that can enhance health , is beyond any doubt one of the leading trends in today 's food industry .
	manualset3
165335	6	412449	7	NULL	NULL	0	NULL	health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for functional foods or functional food ingredients , i.e. foods or food ingredients that can enhance health , is beyond any doubt one of the leading trends in today 's food industry .
	manualset3
165336	7	412449	7	NULL	NULL	0	NULL	leading trends	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for functional foods or functional food ingredients , i.e. foods or food ingredients that can enhance health , is beyond any doubt one of the leading trends in today 's food industry .
	manualset3
165337	8	412449	7	NULL	NULL	0	NULL	 today 's food industry	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for functional foods or functional food ingredients , i.e. foods or food ingredients that can enhance health , is beyond any doubt one of the leading trends in today 's food industry .
	manualset3
165338	1	412450	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our results , single toxicity data derived by the BLM can estimate combined toxicity described as a function of TU .
	manualset3
165339	2	412450	7	NULL	NULL	0	NULL	single toxicity data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our results , single toxicity data derived by the BLM can estimate combined toxicity described as a function of TU .
	manualset3
165340	3	412450	7	NULL	NULL	0	NULL	BLM	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our results , single toxicity data derived by the BLM can estimate combined toxicity described as a function of TU .
	manualset3
165341	4	412450	7	NULL	NULL	0	NULL	 combined toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our results , single toxicity data derived by the BLM can estimate combined toxicity described as a function of TU .
	manualset3
165342	5	412450	7	NULL	NULL	0	NULL	function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our results , single toxicity data derived by the BLM can estimate combined toxicity described as a function of TU .
	manualset3
165343	6	412450	7	NULL	NULL	0	NULL	TU	Unit												NULL		0	NULL	NULL	NULL	NULL	NULL	According to our results , single toxicity data derived by the BLM can estimate combined toxicity described as a function of TU .
	manualset3
165344	1	412451	7	NULL	NULL	0	NULL	search	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for hypercoagulability in these patients led to identification of changes in the expression patterns of coagulation proteins from the coagulation cascade .
	manualset3
165345	2	412451	7	NULL	NULL	0	NULL	hypercoagulability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for hypercoagulability in these patients led to identification of changes in the expression patterns of coagulation proteins from the coagulation cascade .
	manualset3
165346	3	412451	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for hypercoagulability in these patients led to identification of changes in the expression patterns of coagulation proteins from the coagulation cascade .
	manualset3
165347	4	412451	7	NULL	NULL	0	NULL	identification 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for hypercoagulability in these patients led to identification of changes in the expression patterns of coagulation proteins from the coagulation cascade .
	manualset3
165348	5	412451	7	NULL	NULL	0	NULL	changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for hypercoagulability in these patients led to identification of changes in the expression patterns of coagulation proteins from the coagulation cascade .
	manualset3
165349	6	412451	7	NULL	NULL	0	NULL	expression patterns	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for hypercoagulability in these patients led to identification of changes in the expression patterns of coagulation proteins from the coagulation cascade .
	manualset3
165350	7	412451	7	NULL	NULL	0	NULL	coagulation proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for hypercoagulability in these patients led to identification of changes in the expression patterns of coagulation proteins from the coagulation cascade .
	manualset3
165351	8	412451	7	NULL	NULL	NULL	NULL	coagulation cascade	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The search for hypercoagulability in these patients led to identification of changes in the expression patterns of coagulation proteins from the coagulation cascade .
	manualset3
165352	1	412452	7	NULL	NULL	0	NULL	search	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for mechanisms that impose specificity on induction of cell death and NF-kappaB activation by members of the TNF/NGF receptor family .
	manualset3
165353	2	412452	7	NULL	NULL	0	NULL	mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for mechanisms that impose specificity on induction of cell death and NF-kappaB activation by members of the TNF/NGF receptor family .
	manualset3
165354	3	412452	7	NULL	NULL	0	NULL	 induction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for mechanisms that impose specificity on induction of cell death and NF-kappaB activation by members of the TNF/NGF receptor family .
	manualset3
165355	4	412452	7	NULL	NULL	0	NULL	 cell death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for mechanisms that impose specificity on induction of cell death and NF-kappaB activation by members of the TNF/NGF receptor family .
	manualset3
165356	5	412452	7	NULL	NULL	0	NULL	NF-kappaB activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for mechanisms that impose specificity on induction of cell death and NF-kappaB activation by members of the TNF/NGF receptor family .
	manualset3
165357	6	412452	7	NULL	NULL	0	NULL	 members	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for mechanisms that impose specificity on induction of cell death and NF-kappaB activation by members of the TNF/NGF receptor family .
	manualset3
165358	7	412452	7	NULL	NULL	0	NULL	 TNF/NGF receptor family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for mechanisms that impose specificity on induction of cell death and NF-kappaB activation by members of the TNF/NGF receptor family .
	manualset3
166503	8	412452	7	NULL	NULL	NULL	NULL	specificity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The search for mechanisms that impose specificity on induction of cell death and NF-kappaB activation by members of the TNF/NGF receptor family .
	manualset3
165359	1	412453	7	NULL	NULL	0	NULL	search	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for more effective drugs for the treatment of leishmaniasis and trypanosomiasis has increasingly involved the use of in vitro screens .
	manualset3
165360	2	412453	7	NULL	NULL	0	NULL	effective drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for more effective drugs for the treatment of leishmaniasis and trypanosomiasis has increasingly involved the use of in vitro screens .
	manualset3
165361	3	412453	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for more effective drugs for the treatment of leishmaniasis and trypanosomiasis has increasingly involved the use of in vitro screens .
	manualset3
165362	4	412453	7	NULL	NULL	0	NULL	leishmaniasis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for more effective drugs for the treatment of leishmaniasis and trypanosomiasis has increasingly involved the use of in vitro screens .
	manualset3
165363	5	412453	7	NULL	NULL	0	NULL	trypanosomiasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for more effective drugs for the treatment of leishmaniasis and trypanosomiasis has increasingly involved the use of in vitro screens .
	manualset3
165364	6	412453	7	NULL	NULL	0	NULL	in vitro screens	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for more effective drugs for the treatment of leishmaniasis and trypanosomiasis has increasingly involved the use of in vitro screens .
	manualset3
173643	7	412453	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The search for more effective drugs for the treatment of leishmaniasis and trypanosomiasis has increasingly involved the use of in vitro screens .
	manualset3
165365	1	412454	7	NULL	NULL	0	NULL	 search 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The search was conducted in Medline , EMBASE , and Cochrane Database of systematic reviews .
	manualset3
165366	2	412454	7	NULL	NULL	0	NULL	Medline	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The search was conducted in Medline , EMBASE , and Cochrane Database of systematic reviews .
	manualset3
165367	3	412454	7	NULL	NULL	0	NULL	EMBASE	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The search was conducted in Medline , EMBASE , and Cochrane Database of systematic reviews .
	manualset3
165368	4	412454	7	NULL	NULL	0	NULL	Cochrane Database	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The search was conducted in Medline , EMBASE , and Cochrane Database of systematic reviews .
	manualset3
165369	5	412454	7	NULL	NULL	0	NULL	systematic reviews	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The search was conducted in Medline , EMBASE , and Cochrane Database of systematic reviews .
	manualset3
165370	1	412455	7	NULL	NULL	0	NULL	 second class of proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The second class of proteins identified are those which display a high relative affinity for cisplatin-damaged DNA and a low affinity for undamaged duplex DNA .
	manualset3
165371	2	412455	7	NULL	NULL	0	NULL	high relative affinity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The second class of proteins identified are those which display a high relative affinity for cisplatin-damaged DNA and a low affinity for undamaged duplex DNA .
	manualset3
165372	3	412455	7	NULL	NULL	0	NULL	cisplatin-damaged DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The second class of proteins identified are those which display a high relative affinity for cisplatin-damaged DNA and a low affinity for undamaged duplex DNA .
	manualset3
165373	4	412455	7	NULL	NULL	0	NULL	low affinity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The second class of proteins identified are those which display a high relative affinity for cisplatin-damaged DNA and a low affinity for undamaged duplex DNA .
	manualset3
165374	5	412455	7	NULL	NULL	0	NULL	undamaged duplex DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The second class of proteins identified are those which display a high relative affinity for cisplatin-damaged DNA and a low affinity for undamaged duplex DNA .
	manualset3
165375	1	412456	7	NULL	NULL	0	NULL	 second component 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The second component is a linear function of mucosal Na concentration , is unaffected by lithium , and is apparently not related to net Na transport by the tissue .
	manualset3
165376	2	412456	7	NULL	NULL	0	NULL	 linear function	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The second component is a linear function of mucosal Na concentration , is unaffected by lithium , and is apparently not related to net Na transport by the tissue .
	manualset3
165377	3	412456	7	NULL	NULL	0	NULL	mucosal Na concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The second component is a linear function of mucosal Na concentration , is unaffected by lithium , and is apparently not related to net Na transport by the tissue .
	manualset3
165378	4	412456	7	NULL	NULL	0	NULL	lithium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The second component is a linear function of mucosal Na concentration , is unaffected by lithium , and is apparently not related to net Na transport by the tissue .
	manualset3
165379	5	412456	7	NULL	NULL	0	NULL	Na transport 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The second component is a linear function of mucosal Na concentration , is unaffected by lithium , and is apparently not related to net Na transport by the tissue .
	manualset3
165380	6	412456	7	NULL	NULL	0	NULL	tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The second component is a linear function of mucosal Na concentration , is unaffected by lithium , and is apparently not related to net Na transport by the tissue .
	manualset3
165381	1	412457	7	NULL	NULL	0	NULL	second component	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The second component of the reciprocal synapse , located approximately 1.5 micron from the first , was recognized by a localized accumulation of clear membrane vesicles within the neuronal process and a short membrane profile within the cytoplasm of the adjacent hair cell .
	manualset3
165382	2	412457	7	NULL	NULL	0	NULL	 reciprocal synapse	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The second component of the reciprocal synapse , located approximately 1.5 micron from the first , was recognized by a localized accumulation of clear membrane vesicles within the neuronal process and a short membrane profile within the cytoplasm of the adjacent hair cell .
	manualset3
165383	3	412457	7	NULL	NULL	0	NULL	1.5 micron	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The second component of the reciprocal synapse , located approximately 1.5 micron from the first , was recognized by a localized accumulation of clear membrane vesicles within the neuronal process and a short membrane profile within the cytoplasm of the adjacent hair cell .
	manualset3
165384	4	412457	7	NULL	NULL	0	NULL	first	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The second component of the reciprocal synapse , located approximately 1.5 micron from the first , was recognized by a localized accumulation of clear membrane vesicles within the neuronal process and a short membrane profile within the cytoplasm of the adjacent hair cell .
	manualset3
165385	5	412457	7	NULL	NULL	0	NULL	localized accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The second component of the reciprocal synapse , located approximately 1.5 micron from the first , was recognized by a localized accumulation of clear membrane vesicles within the neuronal process and a short membrane profile within the cytoplasm of the adjacent hair cell .
	manualset3
165386	6	412457	7	NULL	NULL	0	NULL	clear membrane vesicles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The second component of the reciprocal synapse , located approximately 1.5 micron from the first , was recognized by a localized accumulation of clear membrane vesicles within the neuronal process and a short membrane profile within the cytoplasm of the adjacent hair cell .
	manualset3
165387	7	412457	7	NULL	NULL	NULL	NULL	neuronal process 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The second component of the reciprocal synapse , located approximately 1.5 micron from the first , was recognized by a localized accumulation of clear membrane vesicles within the neuronal process and a short membrane profile within the cytoplasm of the adjacent hair cell .
	manualset3
165388	8	412457	7	NULL	NULL	0	NULL	short membrane profile	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The second component of the reciprocal synapse , located approximately 1.5 micron from the first , was recognized by a localized accumulation of clear membrane vesicles within the neuronal process and a short membrane profile within the cytoplasm of the adjacent hair cell .
	manualset3
165389	9	412457	7	NULL	NULL	0	NULL	cytoplasm	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The second component of the reciprocal synapse , located approximately 1.5 micron from the first , was recognized by a localized accumulation of clear membrane vesicles within the neuronal process and a short membrane profile within the cytoplasm of the adjacent hair cell .
	manualset3
165390	10	412457	7	NULL	NULL	0	NULL	adjacent hair cell 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The second component of the reciprocal synapse , located approximately 1.5 micron from the first , was recognized by a localized accumulation of clear membrane vesicles within the neuronal process and a short membrane profile within the cytoplasm of the adjacent hair cell .
	manualset3
165391	1	412458	7	NULL	NULL	0	NULL	second dimension	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The second dimension relates to the social and political function of decision-making and broadens what counts as the relevant ends of decision-making to include such things as maintaining relationships , avoiding organisational burden , generating politically and legally defensible decisions and demonstrating the willingness to care .
	manualset3
165392	2	412458	7	NULL	NULL	0	NULL	social function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The second dimension relates to the social and political function of decision-making and broadens what counts as the relevant ends of decision-making to include such things as maintaining relationships , avoiding organisational burden , generating politically and legally defensible decisions and demonstrating the willingness to care .
	manualset3
165393	3	412458	7	NULL	NULL	0	NULL	political function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The second dimension relates to the social and political function of decision-making and broadens what counts as the relevant ends of decision-making to include such things as maintaining relationships , avoiding organisational burden , generating politically and legally defensible decisions and demonstrating the willingness to care .
	manualset3
165394	4	412458	7	NULL	NULL	0	NULL	decision-making 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The second dimension relates to the social and political function of decision-making and broadens what counts as the relevant ends of decision-making to include such things as maintaining relationships , avoiding organisational burden , generating politically and legally defensible decisions and demonstrating the willingness to care .
	manualset3
165396	6	412458	7	NULL	NULL	0	NULL	decision-making	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The second dimension relates to the social and political function of decision-making and broadens what counts as the relevant ends of decision-making to include such things as maintaining relationships , avoiding organisational burden , generating politically and legally defensible decisions and demonstrating the willingness to care .
	manualset3
165397	7	412458	7	NULL	NULL	0	NULL	 things	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The second dimension relates to the social and political function of decision-making and broadens what counts as the relevant ends of decision-making to include such things as maintaining relationships , avoiding organisational burden , generating politically and legally defensible decisions and demonstrating the willingness to care .
	manualset3
165398	8	412458	7	NULL	NULL	0	NULL	relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The second dimension relates to the social and political function of decision-making and broadens what counts as the relevant ends of decision-making to include such things as maintaining relationships , avoiding organisational burden , generating politically and legally defensible decisions and demonstrating the willingness to care .
	manualset3
165399	9	412458	7	NULL	NULL	0	NULL	organisational burden	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The second dimension relates to the social and political function of decision-making and broadens what counts as the relevant ends of decision-making to include such things as maintaining relationships , avoiding organisational burden , generating politically and legally defensible decisions and demonstrating the willingness to care .
	manualset3
165400	10	412458	7	NULL	NULL	0	NULL	politically and legally defensible decisions	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The second dimension relates to the social and political function of decision-making and broadens what counts as the relevant ends of decision-making to include such things as maintaining relationships , avoiding organisational burden , generating politically and legally defensible decisions and demonstrating the willingness to care .
	manualset3
165402	1	412459	7	NULL	NULL	0	NULL	second messenger	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The second messenger cyclic adenosine 5 ` monophosphate ( cAMP ) has been implicated in controlling meiotic maturation .
	manualset3
165403	2	412459	7	NULL	NULL	0	NULL	cyclic adenosine 5 ` monophosphate ( cAMP )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The second messenger cyclic adenosine 5 ` monophosphate ( cAMP ) has been implicated in controlling meiotic maturation .
	manualset3
165404	3	412459	7	NULL	NULL	0	NULL	meiotic maturation .	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The second messenger cyclic adenosine 5 ` monophosphate ( cAMP ) has been implicated in controlling meiotic maturation .
	manualset3
165405	1	412460	7	NULL	NULL	0	NULL	resistance factor	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	According to resistance factor , all P. infestans isolates were sensitive to dimethomorph , cymoxanil , mancozeb and zoxamide , 58.3 % of isolates were sensitive to azoxystrobin and 50 % to metalaxyl .
	manualset3
165406	2	412460	7	NULL	NULL	0	NULL	P. infestans isolates	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	According to resistance factor , all P. infestans isolates were sensitive to dimethomorph , cymoxanil , mancozeb and zoxamide , 58.3 % of isolates were sensitive to azoxystrobin and 50 % to metalaxyl .
	manualset3
165407	3	412460	7	NULL	NULL	0	NULL	dimethomorph	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	According to resistance factor , all P. infestans isolates were sensitive to dimethomorph , cymoxanil , mancozeb and zoxamide , 58.3 % of isolates were sensitive to azoxystrobin and 50 % to metalaxyl .
	manualset3
165408	4	412460	7	NULL	NULL	0	NULL	cymoxanil	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	According to resistance factor , all P. infestans isolates were sensitive to dimethomorph , cymoxanil , mancozeb and zoxamide , 58.3 % of isolates were sensitive to azoxystrobin and 50 % to metalaxyl .
	manualset3
165409	5	412460	7	NULL	NULL	0	NULL	mancozeb	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	According to resistance factor , all P. infestans isolates were sensitive to dimethomorph , cymoxanil , mancozeb and zoxamide , 58.3 % of isolates were sensitive to azoxystrobin and 50 % to metalaxyl .
	manualset3
165410	6	412460	7	NULL	NULL	0	NULL	zoxamide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	According to resistance factor , all P. infestans isolates were sensitive to dimethomorph , cymoxanil , mancozeb and zoxamide , 58.3 % of isolates were sensitive to azoxystrobin and 50 % to metalaxyl .
	manualset3
165411	7	412460	7	NULL	NULL	0	NULL	58.3 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	According to resistance factor , all P. infestans isolates were sensitive to dimethomorph , cymoxanil , mancozeb and zoxamide , 58.3 % of isolates were sensitive to azoxystrobin and 50 % to metalaxyl .
	manualset3
165412	8	412460	7	NULL	NULL	0	NULL	isolates	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	According to resistance factor , all P. infestans isolates were sensitive to dimethomorph , cymoxanil , mancozeb and zoxamide , 58.3 % of isolates were sensitive to azoxystrobin and 50 % to metalaxyl .
	manualset3
165413	9	412460	7	NULL	NULL	0	NULL	azoxystrobin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	According to resistance factor , all P. infestans isolates were sensitive to dimethomorph , cymoxanil , mancozeb and zoxamide , 58.3 % of isolates were sensitive to azoxystrobin and 50 % to metalaxyl .
	manualset3
165414	10	412460	7	NULL	NULL	0	NULL	50 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	According to resistance factor , all P. infestans isolates were sensitive to dimethomorph , cymoxanil , mancozeb and zoxamide , 58.3 % of isolates were sensitive to azoxystrobin and 50 % to metalaxyl .
	manualset3
165415	11	412460	7	NULL	NULL	0	NULL	metalaxyl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	According to resistance factor , all P. infestans isolates were sensitive to dimethomorph , cymoxanil , mancozeb and zoxamide , 58.3 % of isolates were sensitive to azoxystrobin and 50 % to metalaxyl .
	manualset3
165416	1	412461	7	NULL	NULL	0	NULL	second part of the paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The second part of the paper details the varieties of Janetian therapeutic treatments of these disorders : the `` liquidation '' of fixed ideas by hypnosis and suggestion , confrontation techniques , which resemble contemporary cognitive behavioural approaches , and special cognitive ( `` logagogic '' ) interventions .
	manualset3
165417	2	412461	7	NULL	NULL	0	NULL	Janetian therapeutic treatments	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The second part of the paper details the varieties of Janetian therapeutic treatments of these disorders : the `` liquidation '' of fixed ideas by hypnosis and suggestion , confrontation techniques , which resemble contemporary cognitive behavioural approaches , and special cognitive ( `` logagogic '' ) interventions .
	manualset3
165418	3	412461	7	NULL	NULL	0	NULL	disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The second part of the paper details the varieties of Janetian therapeutic treatments of these disorders : the `` liquidation '' of fixed ideas by hypnosis and suggestion , confrontation techniques , which resemble contemporary cognitive behavioural approaches , and special cognitive ( `` logagogic '' ) interventions .
	manualset3
165419	4	412461	7	NULL	NULL	0	NULL	liquidation	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The second part of the paper details the varieties of Janetian therapeutic treatments of these disorders : the `` liquidation '' of fixed ideas by hypnosis and suggestion , confrontation techniques , which resemble contemporary cognitive behavioural approaches , and special cognitive ( `` logagogic '' ) interventions .
	manualset3
165420	5	412461	7	NULL	NULL	0	NULL	fixed ideas	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The second part of the paper details the varieties of Janetian therapeutic treatments of these disorders : the `` liquidation '' of fixed ideas by hypnosis and suggestion , confrontation techniques , which resemble contemporary cognitive behavioural approaches , and special cognitive ( `` logagogic '' ) interventions .
	manualset3
165421	6	412461	7	NULL	NULL	0	NULL	 hypnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The second part of the paper details the varieties of Janetian therapeutic treatments of these disorders : the `` liquidation '' of fixed ideas by hypnosis and suggestion , confrontation techniques , which resemble contemporary cognitive behavioural approaches , and special cognitive ( `` logagogic '' ) interventions .
	manualset3
165422	7	412461	7	NULL	NULL	NULL	NULL	confrontation techniques	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The second part of the paper details the varieties of Janetian therapeutic treatments of these disorders : the `` liquidation '' of fixed ideas by hypnosis and suggestion , confrontation techniques , which resemble contemporary cognitive behavioural approaches , and special cognitive ( `` logagogic '' ) interventions .
	manualset3
165423	8	412461	7	NULL	NULL	NULL	NULL	cognitive behavioural approaches	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The second part of the paper details the varieties of Janetian therapeutic treatments of these disorders : the `` liquidation '' of fixed ideas by hypnosis and suggestion , confrontation techniques , which resemble contemporary cognitive behavioural approaches , and special cognitive ( `` logagogic '' ) interventions .
	manualset3
165424	9	412461	7	NULL	NULL	NULL	NULL	special cognitive ( `` logagogic '' ) interventions	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The second part of the paper details the varieties of Janetian therapeutic treatments of these disorders : the `` liquidation '' of fixed ideas by hypnosis and suggestion , confrontation techniques , which resemble contemporary cognitive behavioural approaches , and special cognitive ( `` logagogic '' ) interventions .
	manualset3
165425	1	412462	7	NULL	NULL	0	NULL	second part of the research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The second part of the research describes in detail indigenous practices of traditional medicine for healing trachoma and other eye diseases , inflammation that were prevalent in Mandatory Palestine .
	manualset3
165426	2	412462	7	NULL	NULL	0	NULL	 indigenous practices	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The second part of the research describes in detail indigenous practices of traditional medicine for healing trachoma and other eye diseases , inflammation that were prevalent in Mandatory Palestine .
	manualset3
165427	3	412462	7	NULL	NULL	0	NULL	traditional medicine	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The second part of the research describes in detail indigenous practices of traditional medicine for healing trachoma and other eye diseases , inflammation that were prevalent in Mandatory Palestine .
	manualset3
165428	4	412462	7	NULL	NULL	0	NULL	trachoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The second part of the research describes in detail indigenous practices of traditional medicine for healing trachoma and other eye diseases , inflammation that were prevalent in Mandatory Palestine .
	manualset3
165429	5	412462	7	NULL	NULL	0	NULL	eye diseases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The second part of the research describes in detail indigenous practices of traditional medicine for healing trachoma and other eye diseases , inflammation that were prevalent in Mandatory Palestine .
	manualset3
165430	6	412462	7	NULL	NULL	0	NULL	inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The second part of the research describes in detail indigenous practices of traditional medicine for healing trachoma and other eye diseases , inflammation that were prevalent in Mandatory Palestine .
	manualset3
165431	7	412462	7	NULL	NULL	0	NULL	Mandatory Palestine 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The second part of the research describes in detail indigenous practices of traditional medicine for healing trachoma and other eye diseases , inflammation that were prevalent in Mandatory Palestine .
	manualset3
165432	1	412463	7	NULL	NULL	0	NULL	 second structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The second structure , whose crystals were prepared by co-crystallization with CP , has been refined at 2.6 A resolution to a crystallographic R factor of 20.2 % .
	manualset3
165433	2	412463	7	NULL	NULL	NULL	NULL	crystals	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The second structure , whose crystals were prepared by co-crystallization with CP , has been refined at 2.6 A resolution to a crystallographic R factor of 20.2 % .
	manualset3
165434	3	412463	7	NULL	NULL	0	NULL	co-crystallization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The second structure , whose crystals were prepared by co-crystallization with CP , has been refined at 2.6 A resolution to a crystallographic R factor of 20.2 % .
	manualset3
165435	4	412463	7	NULL	NULL	0	NULL	CP 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The second structure , whose crystals were prepared by co-crystallization with CP , has been refined at 2.6 A resolution to a crystallographic R factor of 20.2 % .
	manualset3
165436	5	412463	7	NULL	NULL	0	NULL	2.6 A resolution	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The second structure , whose crystals were prepared by co-crystallization with CP , has been refined at 2.6 A resolution to a crystallographic R factor of 20.2 % .
	manualset3
165437	6	412463	7	NULL	NULL	0	NULL	crystallographic R factor	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The second structure , whose crystals were prepared by co-crystallization with CP , has been refined at 2.6 A resolution to a crystallographic R factor of 20.2 % .
	manualset3
165438	7	412463	7	NULL	NULL	0	NULL	20.2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The second structure , whose crystals were prepared by co-crystallization with CP , has been refined at 2.6 A resolution to a crystallographic R factor of 20.2 % .
	manualset3
165439	1	412464	7	NULL	NULL	NULL	NULL	second	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The second shows that this signal is necessary for this alteration because inactivation of the corollary reduces the compensation by frontal-cortex neurons .
	manualset3
165440	2	412464	7	NULL	NULL	NULL	NULL	signal 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The second shows that this signal is necessary for this alteration because inactivation of the corollary reduces the compensation by frontal-cortex neurons .
	manualset3
165441	3	412464	7	NULL	NULL	NULL	NULL	alteration	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The second shows that this signal is necessary for this alteration because inactivation of the corollary reduces the compensation by frontal-cortex neurons .
	manualset3
165442	4	412464	7	NULL	NULL	0	NULL	inactivation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The second shows that this signal is necessary for this alteration because inactivation of the corollary reduces the compensation by frontal-cortex neurons .
	manualset3
165443	5	412464	7	NULL	NULL	0	NULL	corollary	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The second shows that this signal is necessary for this alteration because inactivation of the corollary reduces the compensation by frontal-cortex neurons .
	manualset3
165444	6	412464	7	NULL	NULL	0	NULL	compensation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The second shows that this signal is necessary for this alteration because inactivation of the corollary reduces the compensation by frontal-cortex neurons .
	manualset3
165445	7	412464	7	NULL	NULL	NULL	NULL	frontal-cortex neurons	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The second shows that this signal is necessary for this alteration because inactivation of the corollary reduces the compensation by frontal-cortex neurons .
	manualset3
165446	1	412465	7	NULL	NULL	0	NULL	secondary immune response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The secondary and tertiary immune responses to TNP-KLH and the autoanti-immunoglobulin response were studied in 1 - , 3 - and 6-month-old 129/J and 129/Sv mice .
	manualset3
165447	2	412465	7	NULL	NULL	0	NULL	tertiary immune response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The secondary and tertiary immune responses to TNP-KLH and the autoanti-immunoglobulin response were studied in 1 - , 3 - and 6-month-old 129/J and 129/Sv mice .
	manualset3
165448	3	412465	7	NULL	NULL	0	NULL	TNP-KLH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The secondary and tertiary immune responses to TNP-KLH and the autoanti-immunoglobulin response were studied in 1 - , 3 - and 6-month-old 129/J and 129/Sv mice .
	manualset3
165449	4	412465	7	NULL	NULL	0	NULL	autoanti-immunoglobulin response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The secondary and tertiary immune responses to TNP-KLH and the autoanti-immunoglobulin response were studied in 1 - , 3 - and 6-month-old 129/J and 129/Sv mice .
	manualset3
165450	5	412465	7	NULL	NULL	0	NULL	1 -month-old 129/J and 129/Sv mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The secondary and tertiary immune responses to TNP-KLH and the autoanti-immunoglobulin response were studied in 1 - , 3 - and 6-month-old 129/J and 129/Sv mice .
	manualset3
165451	6	412465	7	NULL	NULL	0	NULL	3 -month-old 129/J and 129/Sv mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The secondary and tertiary immune responses to TNP-KLH and the autoanti-immunoglobulin response were studied in 1 - , 3 - and 6-month-old 129/J and 129/Sv mice .
	manualset3
165452	7	412465	7	NULL	NULL	0	NULL	6-month-old 129/J and 129/Sv mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The secondary and tertiary immune responses to TNP-KLH and the autoanti-immunoglobulin response were studied in 1 - , 3 - and 6-month-old 129/J and 129/Sv mice .
	manualset3
165453	1	412466	7	NULL	NULL	NULL	NULL	secondary ion mass spectrometry ( SIMS ) microscope	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The secondary ion mass spectrometry ( SIMS ) microscope is able to map chemical elements in tissue sections .
	manualset3
165454	2	412466	7	NULL	NULL	0	NULL	chemical elements	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The secondary ion mass spectrometry ( SIMS ) microscope is able to map chemical elements in tissue sections .
	manualset3
165455	3	412466	7	NULL	NULL	0	NULL	tissue sections	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The secondary ion mass spectrometry ( SIMS ) microscope is able to map chemical elements in tissue sections .
	manualset3
165456	1	412467	7	NULL	NULL	0	NULL	sedimentation velocities ( S20 , w )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The sedimentation velocities ( S20 , w ) were 4.1 and 26.5 S , respectively .
	manualset3
165457	2	412467	7	NULL	NULL	0	NULL	4.1 S	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The sedimentation velocities ( S20 , w ) were 4.1 and 26.5 S , respectively .
	manualset3
165458	3	412467	7	NULL	NULL	0	NULL	26.5 S	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The sedimentation velocities ( S20 , w ) were 4.1 and 26.5 S , respectively .
	manualset3
165459	1	412468	7	NULL	NULL	NULL	NULL	segmentation target	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The segmentation target therefore is driven by two forces to smooth the derived optimal bias field and improve the accuracy of the segmentation task .
	manualset3
165460	2	412468	7	NULL	NULL	0	NULL	two forces	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The segmentation target therefore is driven by two forces to smooth the derived optimal bias field and improve the accuracy of the segmentation task .
	manualset3
165461	3	412468	7	NULL	NULL	0	NULL	derived optimal bias field 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The segmentation target therefore is driven by two forces to smooth the derived optimal bias field and improve the accuracy of the segmentation task .
	manualset3
165462	4	412468	7	NULL	NULL	0	NULL	accuracy	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The segmentation target therefore is driven by two forces to smooth the derived optimal bias field and improve the accuracy of the segmentation task .
	manualset3
165463	5	412468	7	NULL	NULL	0	NULL	segmentation task	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The segmentation target therefore is driven by two forces to smooth the derived optimal bias field and improve the accuracy of the segmentation task .
	manualset3
165464	1	412469	7	NULL	NULL	0	NULL	selection 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The selection of a panel of killer yeasts , able to display their activity against reference sensitive yeast isolates under anaerobic conditions in a medium that favored the growth of anaerobes , allowed the use of the killer system to type Bacteroides fragilis isolates for epidemiological purposes .
	manualset3
165465	2	412469	7	NULL	NULL	0	NULL	 panel of killer yeasts	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The selection of a panel of killer yeasts , able to display their activity against reference sensitive yeast isolates under anaerobic conditions in a medium that favored the growth of anaerobes , allowed the use of the killer system to type Bacteroides fragilis isolates for epidemiological purposes .
	manualset3
165466	3	412469	7	NULL	NULL	0	NULL	reference sensitive yeast isolates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The selection of a panel of killer yeasts , able to display their activity against reference sensitive yeast isolates under anaerobic conditions in a medium that favored the growth of anaerobes , allowed the use of the killer system to type Bacteroides fragilis isolates for epidemiological purposes .
	manualset3
165467	4	412469	7	NULL	NULL	0	NULL	anaerobic conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The selection of a panel of killer yeasts , able to display their activity against reference sensitive yeast isolates under anaerobic conditions in a medium that favored the growth of anaerobes , allowed the use of the killer system to type Bacteroides fragilis isolates for epidemiological purposes .
	manualset3
165468	5	412469	7	NULL	NULL	0	NULL	medium	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The selection of a panel of killer yeasts , able to display their activity against reference sensitive yeast isolates under anaerobic conditions in a medium that favored the growth of anaerobes , allowed the use of the killer system to type Bacteroides fragilis isolates for epidemiological purposes .
	manualset3
165469	6	412469	7	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The selection of a panel of killer yeasts , able to display their activity against reference sensitive yeast isolates under anaerobic conditions in a medium that favored the growth of anaerobes , allowed the use of the killer system to type Bacteroides fragilis isolates for epidemiological purposes .
	manualset3
165470	7	412469	7	NULL	NULL	0	NULL	anaerobes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The selection of a panel of killer yeasts , able to display their activity against reference sensitive yeast isolates under anaerobic conditions in a medium that favored the growth of anaerobes , allowed the use of the killer system to type Bacteroides fragilis isolates for epidemiological purposes .
	manualset3
165471	8	412469	7	NULL	NULL	0	NULL	killer system	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The selection of a panel of killer yeasts , able to display their activity against reference sensitive yeast isolates under anaerobic conditions in a medium that favored the growth of anaerobes , allowed the use of the killer system to type Bacteroides fragilis isolates for epidemiological purposes .
	manualset3
165472	9	412469	7	NULL	NULL	0	NULL	Bacteroides fragilis isolates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The selection of a panel of killer yeasts , able to display their activity against reference sensitive yeast isolates under anaerobic conditions in a medium that favored the growth of anaerobes , allowed the use of the killer system to type Bacteroides fragilis isolates for epidemiological purposes .
	manualset3
165473	10	412469	7	NULL	NULL	0	NULL	epidemiological purposes	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The selection of a panel of killer yeasts , able to display their activity against reference sensitive yeast isolates under anaerobic conditions in a medium that favored the growth of anaerobes , allowed the use of the killer system to type Bacteroides fragilis isolates for epidemiological purposes .
	manualset3
173644	11	412469	7	NULL	NULL	0	NULL	activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The selection of a panel of killer yeasts , able to display their activity against reference sensitive yeast isolates under anaerobic conditions in a medium that favored the growth of anaerobes , allowed the use of the killer system to type Bacteroides fragilis isolates for epidemiological purposes .
	manualset3
165474	1	412470	7	NULL	NULL	0	NULL	selection 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The selection of second-line drugs may vary between protocols .
	manualset3
165475	2	412470	7	NULL	NULL	0	NULL	second-line drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The selection of second-line drugs may vary between protocols .
	manualset3
165476	3	412470	7	NULL	NULL	0	NULL	protocols	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The selection of second-line drugs may vary between protocols .
	manualset3
165477	1	412471	7	NULL	NULL	0	NULL	selective alpha 1-adrenoceptor agonist phenylephrine	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The selective alpha 1-adrenoceptor agonist phenylephrine ( 0.3-100 microgram ) given by intra-arterial injection ( i.a. ) into the superior mesenteric artery of the anaesthetized dog produced a decrease in mesenteric blood flow which was preferentially blocked by the alpha 1-adrenoceptor antagonist prazosin ( 30-300 microgram/kg i.v. ) .
	manualset3
165478	2	412471	7	NULL	NULL	0	NULL	 0.3-100 microgram	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The selective alpha 1-adrenoceptor agonist phenylephrine ( 0.3-100 microgram ) given by intra-arterial injection ( i.a. ) into the superior mesenteric artery of the anaesthetized dog produced a decrease in mesenteric blood flow which was preferentially blocked by the alpha 1-adrenoceptor antagonist prazosin ( 30-300 microgram/kg i.v. ) .
	manualset3
165479	3	412471	7	NULL	NULL	0	NULL	intra-arterial injection ( i.a. )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The selective alpha 1-adrenoceptor agonist phenylephrine ( 0.3-100 microgram ) given by intra-arterial injection ( i.a. ) into the superior mesenteric artery of the anaesthetized dog produced a decrease in mesenteric blood flow which was preferentially blocked by the alpha 1-adrenoceptor antagonist prazosin ( 30-300 microgram/kg i.v. ) .
	manualset3
165480	4	412471	7	NULL	NULL	0	NULL	superior mesenteric artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The selective alpha 1-adrenoceptor agonist phenylephrine ( 0.3-100 microgram ) given by intra-arterial injection ( i.a. ) into the superior mesenteric artery of the anaesthetized dog produced a decrease in mesenteric blood flow which was preferentially blocked by the alpha 1-adrenoceptor antagonist prazosin ( 30-300 microgram/kg i.v. ) .
	manualset3
165481	5	412471	7	NULL	NULL	0	NULL	anaesthetized dog	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The selective alpha 1-adrenoceptor agonist phenylephrine ( 0.3-100 microgram ) given by intra-arterial injection ( i.a. ) into the superior mesenteric artery of the anaesthetized dog produced a decrease in mesenteric blood flow which was preferentially blocked by the alpha 1-adrenoceptor antagonist prazosin ( 30-300 microgram/kg i.v. ) .
	manualset3
165482	6	412471	7	NULL	NULL	0	NULL	decrease	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The selective alpha 1-adrenoceptor agonist phenylephrine ( 0.3-100 microgram ) given by intra-arterial injection ( i.a. ) into the superior mesenteric artery of the anaesthetized dog produced a decrease in mesenteric blood flow which was preferentially blocked by the alpha 1-adrenoceptor antagonist prazosin ( 30-300 microgram/kg i.v. ) .
	manualset3
165483	7	412471	7	NULL	NULL	0	NULL	mesenteric blood flow	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The selective alpha 1-adrenoceptor agonist phenylephrine ( 0.3-100 microgram ) given by intra-arterial injection ( i.a. ) into the superior mesenteric artery of the anaesthetized dog produced a decrease in mesenteric blood flow which was preferentially blocked by the alpha 1-adrenoceptor antagonist prazosin ( 30-300 microgram/kg i.v. ) .
	manualset3
165484	8	412471	7	NULL	NULL	0	NULL	alpha 1-adrenoceptor antagonist	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The selective alpha 1-adrenoceptor agonist phenylephrine ( 0.3-100 microgram ) given by intra-arterial injection ( i.a. ) into the superior mesenteric artery of the anaesthetized dog produced a decrease in mesenteric blood flow which was preferentially blocked by the alpha 1-adrenoceptor antagonist prazosin ( 30-300 microgram/kg i.v. ) .
	manualset3
165485	9	412471	7	NULL	NULL	0	NULL	prazosin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The selective alpha 1-adrenoceptor agonist phenylephrine ( 0.3-100 microgram ) given by intra-arterial injection ( i.a. ) into the superior mesenteric artery of the anaesthetized dog produced a decrease in mesenteric blood flow which was preferentially blocked by the alpha 1-adrenoceptor antagonist prazosin ( 30-300 microgram/kg i.v. ) .
	manualset3
165486	10	412471	7	NULL	NULL	0	NULL	30-300 microgram/kg i.v.	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The selective alpha 1-adrenoceptor agonist phenylephrine ( 0.3-100 microgram ) given by intra-arterial injection ( i.a. ) into the superior mesenteric artery of the anaesthetized dog produced a decrease in mesenteric blood flow which was preferentially blocked by the alpha 1-adrenoceptor antagonist prazosin ( 30-300 microgram/kg i.v. ) .
	manualset3
165487	1	412472	7	NULL	NULL	0	NULL	selective kinase inhibition profile 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The selective kinase inhibition profile and the preclinical antitumor activity of R547 suggest that it may be promising for development for use in the treatment of solid tumors .
	manualset3
165488	2	412472	7	NULL	NULL	0	NULL	preclinical antitumor activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The selective kinase inhibition profile and the preclinical antitumor activity of R547 suggest that it may be promising for development for use in the treatment of solid tumors .
	manualset3
165489	3	412472	7	NULL	NULL	0	NULL	R547	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The selective kinase inhibition profile and the preclinical antitumor activity of R547 suggest that it may be promising for development for use in the treatment of solid tumors .
	manualset3
165490	4	412472	7	NULL	NULL	0	NULL	development 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The selective kinase inhibition profile and the preclinical antitumor activity of R547 suggest that it may be promising for development for use in the treatment of solid tumors .
	manualset3
165491	5	412472	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The selective kinase inhibition profile and the preclinical antitumor activity of R547 suggest that it may be promising for development for use in the treatment of solid tumors .
	manualset3
165492	6	412472	7	NULL	NULL	NULL	NULL	solid tumors	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The selective kinase inhibition profile and the preclinical antitumor activity of R547 suggest that it may be promising for development for use in the treatment of solid tumors .
	manualset3
165493	1	412473	7	NULL	NULL	0	NULL	selectivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The selectivity and the sensitivity of the two protein-based biosensors were measured and compared for copper , cadmium , mercury , and zinc ions .
	manualset3
165494	2	412473	7	NULL	NULL	0	NULL	sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The selectivity and the sensitivity of the two protein-based biosensors were measured and compared for copper , cadmium , mercury , and zinc ions .
	manualset3
165495	3	412473	7	NULL	NULL	0	NULL	two protein-based biosensors	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The selectivity and the sensitivity of the two protein-based biosensors were measured and compared for copper , cadmium , mercury , and zinc ions .
	manualset3
165496	4	412473	7	NULL	NULL	0	NULL	copper ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The selectivity and the sensitivity of the two protein-based biosensors were measured and compared for copper , cadmium , mercury , and zinc ions .
	manualset3
165497	5	412473	7	NULL	NULL	0	NULL	cadmium ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The selectivity and the sensitivity of the two protein-based biosensors were measured and compared for copper , cadmium , mercury , and zinc ions .
	manualset3
165498	6	412473	7	NULL	NULL	0	NULL	mercury ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The selectivity and the sensitivity of the two protein-based biosensors were measured and compared for copper , cadmium , mercury , and zinc ions .
	manualset3
165499	7	412473	7	NULL	NULL	0	NULL	zinc ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The selectivity and the sensitivity of the two protein-based biosensors were measured and compared for copper , cadmium , mercury , and zinc ions .
	manualset3
165500	1	412474	7	NULL	NULL	0	NULL	selectivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The selectivity has been shown on the basis of the changes observed in the emission and absorption spectral studies through the removal of Zn ( 2 + ) from ( ZnL ( 2 ) ) by PPi .
	manualset3
165501	2	412474	7	NULL	NULL	NULL	NULL	basis	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The selectivity has been shown on the basis of the changes observed in the emission and absorption spectral studies through the removal of Zn ( 2 + ) from ( ZnL ( 2 ) ) by PPi .
	manualset3
165502	3	412474	7	NULL	NULL	0	NULL	emission spectral studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The selectivity has been shown on the basis of the changes observed in the emission and absorption spectral studies through the removal of Zn ( 2 + ) from ( ZnL ( 2 ) ) by PPi .
	manualset3
165503	4	412474	7	NULL	NULL	0	NULL	absorption spectral studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The selectivity has been shown on the basis of the changes observed in the emission and absorption spectral studies through the removal of Zn ( 2 + ) from ( ZnL ( 2 ) ) by PPi .
	manualset3
165504	5	412474	7	NULL	NULL	0	NULL	removal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The selectivity has been shown on the basis of the changes observed in the emission and absorption spectral studies through the removal of Zn ( 2 + ) from ( ZnL ( 2 ) ) by PPi .
	manualset3
165505	6	412474	7	NULL	NULL	0	NULL	Zn ( 2 + )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The selectivity has been shown on the basis of the changes observed in the emission and absorption spectral studies through the removal of Zn ( 2 + ) from ( ZnL ( 2 ) ) by PPi .
	manualset3
165506	7	412474	7	NULL	NULL	0	NULL	 ZnL ( 2 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The selectivity has been shown on the basis of the changes observed in the emission and absorption spectral studies through the removal of Zn ( 2 + ) from ( ZnL ( 2 ) ) by PPi .
	manualset3
165507	8	412474	7	NULL	NULL	0	NULL	PPi	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The selectivity has been shown on the basis of the changes observed in the emission and absorption spectral studies through the removal of Zn ( 2 + ) from ( ZnL ( 2 ) ) by PPi .
	manualset3
165508	1	412475	7	NULL	NULL	0	NULL	self reported prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The self reported prevalence of valvular heart disease and coronary artery disease was low .
	manualset3
165509	2	412475	7	NULL	NULL	0	NULL	valvular heart disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The self reported prevalence of valvular heart disease and coronary artery disease was low .
	manualset3
165510	3	412475	7	NULL	NULL	0	NULL	coronary artery disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The self reported prevalence of valvular heart disease and coronary artery disease was low .
	manualset3
165511	1	412476	7	NULL	NULL	0	NULL	senescence 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The senescence was characterized by a dose - and time-dependent increase in senescence-associated beta-galactosidase activity , senescence-associated changes in cell morphology , an increase in cell size and lysosomal mass , accumulation of lipofuscin , overexpression of p21 ( CIP1/WAF1/Sdi1 ) protein , and irreversible growth arrest .
	manualset3
165512	2	412476	7	NULL	NULL	NULL	NULL	dose -dependent increase	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The senescence was characterized by a dose - and time-dependent increase in senescence-associated beta-galactosidase activity , senescence-associated changes in cell morphology , an increase in cell size and lysosomal mass , accumulation of lipofuscin , overexpression of p21 ( CIP1/WAF1/Sdi1 ) protein , and irreversible growth arrest .
	manualset3
165513	3	412476	7	NULL	NULL	0	NULL	senescence-associated beta-galactosidase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The senescence was characterized by a dose - and time-dependent increase in senescence-associated beta-galactosidase activity , senescence-associated changes in cell morphology , an increase in cell size and lysosomal mass , accumulation of lipofuscin , overexpression of p21 ( CIP1/WAF1/Sdi1 ) protein , and irreversible growth arrest .
	manualset3
165514	4	412476	7	NULL	NULL	NULL	NULL	senescence-associated changes	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The senescence was characterized by a dose - and time-dependent increase in senescence-associated beta-galactosidase activity , senescence-associated changes in cell morphology , an increase in cell size and lysosomal mass , accumulation of lipofuscin , overexpression of p21 ( CIP1/WAF1/Sdi1 ) protein , and irreversible growth arrest .
	manualset3
165515	5	412476	7	NULL	NULL	NULL	NULL	cell morphology	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The senescence was characterized by a dose - and time-dependent increase in senescence-associated beta-galactosidase activity , senescence-associated changes in cell morphology , an increase in cell size and lysosomal mass , accumulation of lipofuscin , overexpression of p21 ( CIP1/WAF1/Sdi1 ) protein , and irreversible growth arrest .
	manualset3
165516	6	412476	7	NULL	NULL	0	NULL	increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The senescence was characterized by a dose - and time-dependent increase in senescence-associated beta-galactosidase activity , senescence-associated changes in cell morphology , an increase in cell size and lysosomal mass , accumulation of lipofuscin , overexpression of p21 ( CIP1/WAF1/Sdi1 ) protein , and irreversible growth arrest .
	manualset3
165517	7	412476	7	NULL	NULL	0	NULL	cell size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The senescence was characterized by a dose - and time-dependent increase in senescence-associated beta-galactosidase activity , senescence-associated changes in cell morphology , an increase in cell size and lysosomal mass , accumulation of lipofuscin , overexpression of p21 ( CIP1/WAF1/Sdi1 ) protein , and irreversible growth arrest .
	manualset3
165518	8	412476	7	NULL	NULL	0	NULL	lysosomal mass	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The senescence was characterized by a dose - and time-dependent increase in senescence-associated beta-galactosidase activity , senescence-associated changes in cell morphology , an increase in cell size and lysosomal mass , accumulation of lipofuscin , overexpression of p21 ( CIP1/WAF1/Sdi1 ) protein , and irreversible growth arrest .
	manualset3
165519	9	412476	7	NULL	NULL	0	NULL	accumulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The senescence was characterized by a dose - and time-dependent increase in senescence-associated beta-galactosidase activity , senescence-associated changes in cell morphology , an increase in cell size and lysosomal mass , accumulation of lipofuscin , overexpression of p21 ( CIP1/WAF1/Sdi1 ) protein , and irreversible growth arrest .
	manualset3
165520	10	412476	7	NULL	NULL	0	NULL	lipofuscin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The senescence was characterized by a dose - and time-dependent increase in senescence-associated beta-galactosidase activity , senescence-associated changes in cell morphology , an increase in cell size and lysosomal mass , accumulation of lipofuscin , overexpression of p21 ( CIP1/WAF1/Sdi1 ) protein , and irreversible growth arrest .
	manualset3
165521	11	412476	7	NULL	NULL	0	NULL	overexpression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The senescence was characterized by a dose - and time-dependent increase in senescence-associated beta-galactosidase activity , senescence-associated changes in cell morphology , an increase in cell size and lysosomal mass , accumulation of lipofuscin , overexpression of p21 ( CIP1/WAF1/Sdi1 ) protein , and irreversible growth arrest .
	manualset3
165522	12	412476	7	NULL	NULL	0	NULL	p21 ( CIP1/WAF1/Sdi1 ) protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The senescence was characterized by a dose - and time-dependent increase in senescence-associated beta-galactosidase activity , senescence-associated changes in cell morphology , an increase in cell size and lysosomal mass , accumulation of lipofuscin , overexpression of p21 ( CIP1/WAF1/Sdi1 ) protein , and irreversible growth arrest .
	manualset3
165523	13	412476	7	NULL	NULL	0	NULL	irreversible growth arrest	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The senescence was characterized by a dose - and time-dependent increase in senescence-associated beta-galactosidase activity , senescence-associated changes in cell morphology , an increase in cell size and lysosomal mass , accumulation of lipofuscin , overexpression of p21 ( CIP1/WAF1/Sdi1 ) protein , and irreversible growth arrest .
	manualset3
166504	14	412476	7	NULL	NULL	0	NULL	time-dependent increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The senescence was characterized by a dose - and time-dependent increase in senescence-associated beta-galactosidase activity , senescence-associated changes in cell morphology , an increase in cell size and lysosomal mass , accumulation of lipofuscin , overexpression of p21 ( CIP1/WAF1/Sdi1 ) protein , and irreversible growth arrest .
	manualset3
165524	1	412477	7	NULL	NULL	NULL	NULL	sensing tests results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The sensing tests results showed that ZnO nanodisks exhibited the greatest sensitivity for the detection of toxic 2-chlorophenol .
	manualset3
165525	2	412477	7	NULL	NULL	0	NULL	 ZnO nanodisks	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensing tests results showed that ZnO nanodisks exhibited the greatest sensitivity for the detection of toxic 2-chlorophenol .
	manualset3
165526	3	412477	7	NULL	NULL	0	NULL	sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensing tests results showed that ZnO nanodisks exhibited the greatest sensitivity for the detection of toxic 2-chlorophenol .
	manualset3
165527	4	412477	7	NULL	NULL	0	NULL	detection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensing tests results showed that ZnO nanodisks exhibited the greatest sensitivity for the detection of toxic 2-chlorophenol .
	manualset3
165528	5	412477	7	NULL	NULL	0	NULL	toxic 2-chlorophenol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensing tests results showed that ZnO nanodisks exhibited the greatest sensitivity for the detection of toxic 2-chlorophenol .
	manualset3
165529	1	412478	7	NULL	NULL	0	NULL	sensitivity ( response/photon )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity ( response/photon ) of distal cells can be modified by background light which passes through a screening pigment found in cells that surround the eye .
	manualset3
165530	2	412478	7	NULL	NULL	0	NULL	distal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity ( response/photon ) of distal cells can be modified by background light which passes through a screening pigment found in cells that surround the eye .
	manualset3
165531	3	412478	7	NULL	NULL	0	NULL	background light	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity ( response/photon ) of distal cells can be modified by background light which passes through a screening pigment found in cells that surround the eye .
	manualset3
165532	4	412478	7	NULL	NULL	0	NULL	screening pigment	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity ( response/photon ) of distal cells can be modified by background light which passes through a screening pigment found in cells that surround the eye .
	manualset3
165533	5	412478	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity ( response/photon ) of distal cells can be modified by background light which passes through a screening pigment found in cells that surround the eye .
	manualset3
165534	6	412478	7	NULL	NULL	0	NULL	 eye	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity ( response/photon ) of distal cells can be modified by background light which passes through a screening pigment found in cells that surround the eye .
	manualset3
165535	1	412479	7	NULL	NULL	NULL	NULL	RTOG scoring system 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	According to the RTOG scoring system 19 irradiated fields with grade II to IV lesions were treated .
	manualset3
165536	2	412479	7	NULL	NULL	0	NULL	19 irradiated fields	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the RTOG scoring system 19 irradiated fields with grade II to IV lesions were treated .
	manualset3
165537	3	412479	7	NULL	NULL	0	NULL	grade II lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the RTOG scoring system 19 irradiated fields with grade II to IV lesions were treated .
	manualset3
165538	4	412479	7	NULL	NULL	0	NULL	grade IV lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the RTOG scoring system 19 irradiated fields with grade II to IV lesions were treated .
	manualset3
165539	1	412480	7	NULL	NULL	0	NULL	sensitivity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity and specificity of the DNA probe for P. micros was 99.2 % and 100 % , respectively .
	manualset3
165540	2	412480	7	NULL	NULL	0	NULL	specificity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity and specificity of the DNA probe for P. micros was 99.2 % and 100 % , respectively .
	manualset3
165541	3	412480	7	NULL	NULL	0	NULL	DNA probe	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity and specificity of the DNA probe for P. micros was 99.2 % and 100 % , respectively .
	manualset3
165542	4	412480	7	NULL	NULL	0	NULL	P. micros	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity and specificity of the DNA probe for P. micros was 99.2 % and 100 % , respectively .
	manualset3
165543	5	412480	7	NULL	NULL	0	NULL	99.2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity and specificity of the DNA probe for P. micros was 99.2 % and 100 % , respectively .
	manualset3
165544	6	412480	7	NULL	NULL	0	NULL	100 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity and specificity of the DNA probe for P. micros was 99.2 % and 100 % , respectively .
	manualset3
165545	1	412481	7	NULL	NULL	0	NULL	sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity and specificity of the colposcopic score for the detection of high-grade lesions for each group were respectively : 87.5 and 92.3 % for NP + patients ; 90.9 and 92 % for NP - patients ; 100 and 87.5 % for P + patients and 100 and 91.7 % for P - patients .
	manualset3
165546	2	412481	7	NULL	NULL	0	NULL	specificity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity and specificity of the colposcopic score for the detection of high-grade lesions for each group were respectively : 87.5 and 92.3 % for NP + patients ; 90.9 and 92 % for NP - patients ; 100 and 87.5 % for P + patients and 100 and 91.7 % for P - patients .
	manualset3
165547	3	412481	7	NULL	NULL	0	NULL	 colposcopic score	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity and specificity of the colposcopic score for the detection of high-grade lesions for each group were respectively : 87.5 and 92.3 % for NP + patients ; 90.9 and 92 % for NP - patients ; 100 and 87.5 % for P + patients and 100 and 91.7 % for P - patients .
	manualset3
165548	4	412481	7	NULL	NULL	0	NULL	high-grade lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity and specificity of the colposcopic score for the detection of high-grade lesions for each group were respectively : 87.5 and 92.3 % for NP + patients ; 90.9 and 92 % for NP - patients ; 100 and 87.5 % for P + patients and 100 and 91.7 % for P - patients .
	manualset3
165549	5	412481	7	NULL	NULL	0	NULL	group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity and specificity of the colposcopic score for the detection of high-grade lesions for each group were respectively : 87.5 and 92.3 % for NP + patients ; 90.9 and 92 % for NP - patients ; 100 and 87.5 % for P + patients and 100 and 91.7 % for P - patients .
	manualset3
165550	6	412481	7	NULL	NULL	0	NULL	 87.5 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity and specificity of the colposcopic score for the detection of high-grade lesions for each group were respectively : 87.5 and 92.3 % for NP + patients ; 90.9 and 92 % for NP - patients ; 100 and 87.5 % for P + patients and 100 and 91.7 % for P - patients .
	manualset3
165551	7	412481	7	NULL	NULL	0	NULL	92.3 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity and specificity of the colposcopic score for the detection of high-grade lesions for each group were respectively : 87.5 and 92.3 % for NP + patients ; 90.9 and 92 % for NP - patients ; 100 and 87.5 % for P + patients and 100 and 91.7 % for P - patients .
	manualset3
165552	8	412481	7	NULL	NULL	0	NULL	NP + patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity and specificity of the colposcopic score for the detection of high-grade lesions for each group were respectively : 87.5 and 92.3 % for NP + patients ; 90.9 and 92 % for NP - patients ; 100 and 87.5 % for P + patients and 100 and 91.7 % for P - patients .
	manualset3
165553	9	412481	7	NULL	NULL	0	NULL	90.9%	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity and specificity of the colposcopic score for the detection of high-grade lesions for each group were respectively : 87.5 and 92.3 % for NP + patients ; 90.9 and 92 % for NP - patients ; 100 and 87.5 % for P + patients and 100 and 91.7 % for P - patients .
	manualset3
165554	10	412481	7	NULL	NULL	0	NULL	 92 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity and specificity of the colposcopic score for the detection of high-grade lesions for each group were respectively : 87.5 and 92.3 % for NP + patients ; 90.9 and 92 % for NP - patients ; 100 and 87.5 % for P + patients and 100 and 91.7 % for P - patients .
	manualset3
165555	11	412481	7	NULL	NULL	0	NULL	NP - patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity and specificity of the colposcopic score for the detection of high-grade lesions for each group were respectively : 87.5 and 92.3 % for NP + patients ; 90.9 and 92 % for NP - patients ; 100 and 87.5 % for P + patients and 100 and 91.7 % for P - patients .
	manualset3
165556	12	412481	7	NULL	NULL	0	NULL	100 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity and specificity of the colposcopic score for the detection of high-grade lesions for each group were respectively : 87.5 and 92.3 % for NP + patients ; 90.9 and 92 % for NP - patients ; 100 and 87.5 % for P + patients and 100 and 91.7 % for P - patients .
	manualset3
165557	13	412481	7	NULL	NULL	0	NULL	87.5 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity and specificity of the colposcopic score for the detection of high-grade lesions for each group were respectively : 87.5 and 92.3 % for NP + patients ; 90.9 and 92 % for NP - patients ; 100 and 87.5 % for P + patients and 100 and 91.7 % for P - patients .
	manualset3
165558	14	412481	7	NULL	NULL	0	NULL	P + patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity and specificity of the colposcopic score for the detection of high-grade lesions for each group were respectively : 87.5 and 92.3 % for NP + patients ; 90.9 and 92 % for NP - patients ; 100 and 87.5 % for P + patients and 100 and 91.7 % for P - patients .
	manualset3
165559	15	412481	7	NULL	NULL	0	NULL	100 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity and specificity of the colposcopic score for the detection of high-grade lesions for each group were respectively : 87.5 and 92.3 % for NP + patients ; 90.9 and 92 % for NP - patients ; 100 and 87.5 % for P + patients and 100 and 91.7 % for P - patients .
	manualset3
165560	16	412481	7	NULL	NULL	0	NULL	91.7 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity and specificity of the colposcopic score for the detection of high-grade lesions for each group were respectively : 87.5 and 92.3 % for NP + patients ; 90.9 and 92 % for NP - patients ; 100 and 87.5 % for P + patients and 100 and 91.7 % for P - patients .
	manualset3
165561	17	412481	7	NULL	NULL	0	NULL	P - patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity and specificity of the colposcopic score for the detection of high-grade lesions for each group were respectively : 87.5 and 92.3 % for NP + patients ; 90.9 and 92 % for NP - patients ; 100 and 87.5 % for P + patients and 100 and 91.7 % for P - patients .
	manualset3
165562	18	412481	7	NULL	NULL	0	NULL	detection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity and specificity of the colposcopic score for the detection of high-grade lesions for each group were respectively : 87.5 and 92.3 % for NP + patients ; 90.9 and 92 % for NP - patients ; 100 and 87.5 % for P + patients and 100 and 91.7 % for P - patients .
	manualset3
165563	1	412482	7	NULL	NULL	0	NULL	sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity of the data was more varied , ranging from 0 to 100 % , reflecting that if a rare condition was present it often was not documented on the birth certificate .
	manualset3
165564	2	412482	7	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity of the data was more varied , ranging from 0 to 100 % , reflecting that if a rare condition was present it often was not documented on the birth certificate .
	manualset3
165565	3	412482	7	NULL	NULL	0	NULL	0 to 100 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity of the data was more varied , ranging from 0 to 100 % , reflecting that if a rare condition was present it often was not documented on the birth certificate .
	manualset3
165566	4	412482	7	NULL	NULL	0	NULL	rare condition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity of the data was more varied , ranging from 0 to 100 % , reflecting that if a rare condition was present it often was not documented on the birth certificate .
	manualset3
165567	5	412482	7	NULL	NULL	0	NULL	birth certificate	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity of the data was more varied , ranging from 0 to 100 % , reflecting that if a rare condition was present it often was not documented on the birth certificate .
	manualset3
165568	1	412483	7	NULL	NULL	0	NULL	 sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity of the method is such that 10 ng of drug can be measured per aliquot of biological fluid .
	manualset3
165569	2	412483	7	NULL	NULL	NULL	NULL	 method	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The sensitivity of the method is such that 10 ng of drug can be measured per aliquot of biological fluid .
	manualset3
165570	3	412483	7	NULL	NULL	0	NULL	10 ng	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity of the method is such that 10 ng of drug can be measured per aliquot of biological fluid .
	manualset3
165571	4	412483	7	NULL	NULL	0	NULL	 drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity of the method is such that 10 ng of drug can be measured per aliquot of biological fluid .
	manualset3
165572	5	412483	7	NULL	NULL	0	NULL	biological fluid	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity of the method is such that 10 ng of drug can be measured per aliquot of biological fluid .
	manualset3
165573	1	412484	7	NULL	NULL	NULL	NULL	sensitivity	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The sensitivity of the procedure is about 15 ng/ml in biological fluid .
	manualset3
165574	2	412484	7	NULL	NULL	0	NULL	procedure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity of the procedure is about 15 ng/ml in biological fluid .
	manualset3
165575	3	412484	7	NULL	NULL	0	NULL	15 ng/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity of the procedure is about 15 ng/ml in biological fluid .
	manualset3
165576	4	412484	7	NULL	NULL	0	NULL	biological fluid	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity of the procedure is about 15 ng/ml in biological fluid .
	manualset3
165577	1	412485	7	NULL	NULL	0	NULL	separation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The separation of proteins from olive oils by CE has been achieved for the first time in this work .
	manualset3
165578	2	412485	7	NULL	NULL	0	NULL	proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The separation of proteins from olive oils by CE has been achieved for the first time in this work .
	manualset3
165579	3	412485	7	NULL	NULL	0	NULL	olive oils	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The separation of proteins from olive oils by CE has been achieved for the first time in this work .
	manualset3
165580	4	412485	7	NULL	NULL	0	NULL	CE	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The separation of proteins from olive oils by CE has been achieved for the first time in this work .
	manualset3
165581	5	412485	7	NULL	NULL	0	NULL	first time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The separation of proteins from olive oils by CE has been achieved for the first time in this work .
	manualset3
165582	6	412485	7	NULL	NULL	0	NULL	 work	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The separation of proteins from olive oils by CE has been achieved for the first time in this work .
	manualset3
165583	1	412486	7	NULL	NULL	0	NULL	separation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The separation was carried out through a gradient elution using an Agilent LiChrospher C18 column ( 250x4 .0 mm id , 5 microm ) and a mobile phase consisting of ( A ) water-TFA ( 99.9 : 0.1 v/v ) and ( B ) acetonitrile-TFA ( 99.1 : 0.1 v/v ) delivered at a flow-rate of 1.0 mL/min .
	manualset3
165584	2	412486	7	NULL	NULL	0	NULL	 gradient elution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The separation was carried out through a gradient elution using an Agilent LiChrospher C18 column ( 250x4 .0 mm id , 5 microm ) and a mobile phase consisting of ( A ) water-TFA ( 99.9 : 0.1 v/v ) and ( B ) acetonitrile-TFA ( 99.1 : 0.1 v/v ) delivered at a flow-rate of 1.0 mL/min .
	manualset3
165585	3	412486	7	NULL	NULL	0	NULL	Agilent LiChrospher C18 column	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The separation was carried out through a gradient elution using an Agilent LiChrospher C18 column ( 250x4 .0 mm id , 5 microm ) and a mobile phase consisting of ( A ) water-TFA ( 99.9 : 0.1 v/v ) and ( B ) acetonitrile-TFA ( 99.1 : 0.1 v/v ) delivered at a flow-rate of 1.0 mL/min .
	manualset3
165586	4	412486	7	NULL	NULL	0	NULL	250x4 .0 mm id , 5 microm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The separation was carried out through a gradient elution using an Agilent LiChrospher C18 column ( 250x4 .0 mm id , 5 microm ) and a mobile phase consisting of ( A ) water-TFA ( 99.9 : 0.1 v/v ) and ( B ) acetonitrile-TFA ( 99.1 : 0.1 v/v ) delivered at a flow-rate of 1.0 mL/min .
	manualset3
165587	5	412486	7	NULL	NULL	0	NULL	mobile phase	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The separation was carried out through a gradient elution using an Agilent LiChrospher C18 column ( 250x4 .0 mm id , 5 microm ) and a mobile phase consisting of ( A ) water-TFA ( 99.9 : 0.1 v/v ) and ( B ) acetonitrile-TFA ( 99.1 : 0.1 v/v ) delivered at a flow-rate of 1.0 mL/min .
	manualset3
165588	6	412486	7	NULL	NULL	0	NULL	 water-TFA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The separation was carried out through a gradient elution using an Agilent LiChrospher C18 column ( 250x4 .0 mm id , 5 microm ) and a mobile phase consisting of ( A ) water-TFA ( 99.9 : 0.1 v/v ) and ( B ) acetonitrile-TFA ( 99.1 : 0.1 v/v ) delivered at a flow-rate of 1.0 mL/min .
	manualset3
165589	7	412486	7	NULL	NULL	0	NULL	99.9 : 0.1 v/v	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The separation was carried out through a gradient elution using an Agilent LiChrospher C18 column ( 250x4 .0 mm id , 5 microm ) and a mobile phase consisting of ( A ) water-TFA ( 99.9 : 0.1 v/v ) and ( B ) acetonitrile-TFA ( 99.1 : 0.1 v/v ) delivered at a flow-rate of 1.0 mL/min .
	manualset3
165590	8	412486	7	NULL	NULL	0	NULL	acetonitrile-TFA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The separation was carried out through a gradient elution using an Agilent LiChrospher C18 column ( 250x4 .0 mm id , 5 microm ) and a mobile phase consisting of ( A ) water-TFA ( 99.9 : 0.1 v/v ) and ( B ) acetonitrile-TFA ( 99.1 : 0.1 v/v ) delivered at a flow-rate of 1.0 mL/min .
	manualset3
165591	9	412486	7	NULL	NULL	0	NULL	99.1 : 0.1 v/v	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The separation was carried out through a gradient elution using an Agilent LiChrospher C18 column ( 250x4 .0 mm id , 5 microm ) and a mobile phase consisting of ( A ) water-TFA ( 99.9 : 0.1 v/v ) and ( B ) acetonitrile-TFA ( 99.1 : 0.1 v/v ) delivered at a flow-rate of 1.0 mL/min .
	manualset3
165592	10	412486	7	NULL	NULL	0	NULL	flow-rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The separation was carried out through a gradient elution using an Agilent LiChrospher C18 column ( 250x4 .0 mm id , 5 microm ) and a mobile phase consisting of ( A ) water-TFA ( 99.9 : 0.1 v/v ) and ( B ) acetonitrile-TFA ( 99.1 : 0.1 v/v ) delivered at a flow-rate of 1.0 mL/min .
	manualset3
165593	11	412486	7	NULL	NULL	0	NULL	1.0 mL/min	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The separation was carried out through a gradient elution using an Agilent LiChrospher C18 column ( 250x4 .0 mm id , 5 microm ) and a mobile phase consisting of ( A ) water-TFA ( 99.9 : 0.1 v/v ) and ( B ) acetonitrile-TFA ( 99.1 : 0.1 v/v ) delivered at a flow-rate of 1.0 mL/min .
	manualset3
165594	1	412487	7	NULL	NULL	0	NULL	sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The sequence at the termini are exactly the same as those at the ends of the native double-stranded RNA gene .
	manualset3
165595	2	412487	7	NULL	NULL	0	NULL	 termini	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The sequence at the termini are exactly the same as those at the ends of the native double-stranded RNA gene .
	manualset3
165596	3	412487	7	NULL	NULL	0	NULL	ends	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The sequence at the termini are exactly the same as those at the ends of the native double-stranded RNA gene .
	manualset3
165597	4	412487	7	NULL	NULL	0	NULL	native double-stranded RNA gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The sequence at the termini are exactly the same as those at the ends of the native double-stranded RNA gene .
	manualset3
165598	1	412488	7	NULL	NULL	0	NULL	sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The sequence in which the pathology appears in the deteriorating fetus is as follows : the first to become non-reactive is the FMAC-test , followed by decreased fetal movements till cessation , and , finally , severe changes in the FHR-NST take place .
	manualset3
165599	2	412488	7	NULL	NULL	0	NULL	pathology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The sequence in which the pathology appears in the deteriorating fetus is as follows : the first to become non-reactive is the FMAC-test , followed by decreased fetal movements till cessation , and , finally , severe changes in the FHR-NST take place .
	manualset3
165600	3	412488	7	NULL	NULL	0	NULL	deteriorating fetus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The sequence in which the pathology appears in the deteriorating fetus is as follows : the first to become non-reactive is the FMAC-test , followed by decreased fetal movements till cessation , and , finally , severe changes in the FHR-NST take place .
	manualset3
165601	4	412488	7	NULL	NULL	0	NULL	first	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The sequence in which the pathology appears in the deteriorating fetus is as follows : the first to become non-reactive is the FMAC-test , followed by decreased fetal movements till cessation , and , finally , severe changes in the FHR-NST take place .
	manualset3
165602	5	412488	7	NULL	NULL	0	NULL	non-reactive	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The sequence in which the pathology appears in the deteriorating fetus is as follows : the first to become non-reactive is the FMAC-test , followed by decreased fetal movements till cessation , and , finally , severe changes in the FHR-NST take place .
	manualset3
165603	6	412488	7	NULL	NULL	0	NULL	FMAC-test	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The sequence in which the pathology appears in the deteriorating fetus is as follows : the first to become non-reactive is the FMAC-test , followed by decreased fetal movements till cessation , and , finally , severe changes in the FHR-NST take place .
	manualset3
165604	7	412488	7	NULL	NULL	0	NULL	decreased fetal movements	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The sequence in which the pathology appears in the deteriorating fetus is as follows : the first to become non-reactive is the FMAC-test , followed by decreased fetal movements till cessation , and , finally , severe changes in the FHR-NST take place .
	manualset3
165605	8	412488	7	NULL	NULL	0	NULL	cessation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The sequence in which the pathology appears in the deteriorating fetus is as follows : the first to become non-reactive is the FMAC-test , followed by decreased fetal movements till cessation , and , finally , severe changes in the FHR-NST take place .
	manualset3
165606	9	412488	7	NULL	NULL	0	NULL	FHR-NST	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The sequence in which the pathology appears in the deteriorating fetus is as follows : the first to become non-reactive is the FMAC-test , followed by decreased fetal movements till cessation , and , finally , severe changes in the FHR-NST take place .
	manualset3
165607	1	412489	7	NULL	NULL	0	NULL	sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The sequence of mouse DNA flanking the insertion site junctions was determined .
	manualset3
165608	2	412489	7	NULL	NULL	0	NULL	mouse DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The sequence of mouse DNA flanking the insertion site junctions was determined .
	manualset3
165609	3	412489	7	NULL	NULL	0	NULL	 insertion site junctions	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The sequence of mouse DNA flanking the insertion site junctions was determined .
	manualset3
165610	1	412490	7	NULL	NULL	0	NULL	sequential treatment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The sequential treatment of AEW followed by CaA ( AEW-CaA ) achieved the best overall dual control of browning and bacterial growth on fresh-cut apple wedges .
	manualset3
165611	2	412490	7	NULL	NULL	0	NULL	AEW	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The sequential treatment of AEW followed by CaA ( AEW-CaA ) achieved the best overall dual control of browning and bacterial growth on fresh-cut apple wedges .
	manualset3
165612	3	412490	7	NULL	NULL	0	NULL	CaA ( AEW-CaA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The sequential treatment of AEW followed by CaA ( AEW-CaA ) achieved the best overall dual control of browning and bacterial growth on fresh-cut apple wedges .
	manualset3
165613	4	412490	7	NULL	NULL	0	NULL	dual control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The sequential treatment of AEW followed by CaA ( AEW-CaA ) achieved the best overall dual control of browning and bacterial growth on fresh-cut apple wedges .
	manualset3
165614	5	412490	7	NULL	NULL	0	NULL	 browning	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The sequential treatment of AEW followed by CaA ( AEW-CaA ) achieved the best overall dual control of browning and bacterial growth on fresh-cut apple wedges .
	manualset3
165615	6	412490	7	NULL	NULL	0	NULL	bacterial growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The sequential treatment of AEW followed by CaA ( AEW-CaA ) achieved the best overall dual control of browning and bacterial growth on fresh-cut apple wedges .
	manualset3
165616	7	412490	7	NULL	NULL	0	NULL	fresh-cut apple wedges 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The sequential treatment of AEW followed by CaA ( AEW-CaA ) achieved the best overall dual control of browning and bacterial growth on fresh-cut apple wedges .
	manualset3
165617	1	412491	7	NULL	NULL	0	NULL	series	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The series of oligosaccharides was completely separated by 7-MPa , liquid chromatography ( l.c. ) on a Micropak NH2-10 column ; the analysis could be performed with isocratic or gradient solvent-systems , and did not involve derivatization .
	manualset3
165618	2	412491	7	NULL	NULL	0	NULL	oligosaccharides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The series of oligosaccharides was completely separated by 7-MPa , liquid chromatography ( l.c. ) on a Micropak NH2-10 column ; the analysis could be performed with isocratic or gradient solvent-systems , and did not involve derivatization .
	manualset3
165619	3	412491	7	NULL	NULL	0	NULL	7-MPa	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The series of oligosaccharides was completely separated by 7-MPa , liquid chromatography ( l.c. ) on a Micropak NH2-10 column ; the analysis could be performed with isocratic or gradient solvent-systems , and did not involve derivatization .
	manualset3
165620	4	412491	7	NULL	NULL	0	NULL	liquid chromatography ( l.c. )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The series of oligosaccharides was completely separated by 7-MPa , liquid chromatography ( l.c. ) on a Micropak NH2-10 column ; the analysis could be performed with isocratic or gradient solvent-systems , and did not involve derivatization .
	manualset3
165621	5	412491	7	NULL	NULL	NULL	NULL	Micropak NH2-10 column	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The series of oligosaccharides was completely separated by 7-MPa , liquid chromatography ( l.c. ) on a Micropak NH2-10 column ; the analysis could be performed with isocratic or gradient solvent-systems , and did not involve derivatization .
	manualset3
165622	6	412491	7	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The series of oligosaccharides was completely separated by 7-MPa , liquid chromatography ( l.c. ) on a Micropak NH2-10 column ; the analysis could be performed with isocratic or gradient solvent-systems , and did not involve derivatization .
	manualset3
165623	7	412491	7	NULL	NULL	0	NULL	isocratic or gradient solvent-systems	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The series of oligosaccharides was completely separated by 7-MPa , liquid chromatography ( l.c. ) on a Micropak NH2-10 column ; the analysis could be performed with isocratic or gradient solvent-systems , and did not involve derivatization .
	manualset3
165624	8	412491	7	NULL	NULL	0	NULL	derivatization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The series of oligosaccharides was completely separated by 7-MPa , liquid chromatography ( l.c. ) on a Micropak NH2-10 column ; the analysis could be performed with isocratic or gradient solvent-systems , and did not involve derivatization .
	manualset3
165625	1	412492	7	NULL	NULL	NULL	NULL	serotonin system	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The serotonin system and NMDA receptors ( NMDARs ) in prefrontal cortex ( PFC ) are both critically involved in the regulation of cognition and emotion under normal and pathological conditions ; however , the interactions between them are essentially unknown .
	manualset3
165626	2	412492	7	NULL	NULL	0	NULL	NMDA receptors ( NMDARs )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The serotonin system and NMDA receptors ( NMDARs ) in prefrontal cortex ( PFC ) are both critically involved in the regulation of cognition and emotion under normal and pathological conditions ; however , the interactions between them are essentially unknown .
	manualset3
165627	3	412492	7	NULL	NULL	0	NULL	prefrontal cortex ( PFC )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The serotonin system and NMDA receptors ( NMDARs ) in prefrontal cortex ( PFC ) are both critically involved in the regulation of cognition and emotion under normal and pathological conditions ; however , the interactions between them are essentially unknown .
	manualset3
165628	4	412492	7	NULL	NULL	0	NULL	regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The serotonin system and NMDA receptors ( NMDARs ) in prefrontal cortex ( PFC ) are both critically involved in the regulation of cognition and emotion under normal and pathological conditions ; however , the interactions between them are essentially unknown .
	manualset3
165629	5	412492	7	NULL	NULL	NULL	NULL	cognition	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The serotonin system and NMDA receptors ( NMDARs ) in prefrontal cortex ( PFC ) are both critically involved in the regulation of cognition and emotion under normal and pathological conditions ; however , the interactions between them are essentially unknown .
	manualset3
165630	6	412492	7	NULL	NULL	NULL	NULL	emotion	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The serotonin system and NMDA receptors ( NMDARs ) in prefrontal cortex ( PFC ) are both critically involved in the regulation of cognition and emotion under normal and pathological conditions ; however , the interactions between them are essentially unknown .
	manualset3
165631	7	412492	7	NULL	NULL	0	NULL	normal conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The serotonin system and NMDA receptors ( NMDARs ) in prefrontal cortex ( PFC ) are both critically involved in the regulation of cognition and emotion under normal and pathological conditions ; however , the interactions between them are essentially unknown .
	manualset3
165632	8	412492	7	NULL	NULL	0	NULL	pathological conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The serotonin system and NMDA receptors ( NMDARs ) in prefrontal cortex ( PFC ) are both critically involved in the regulation of cognition and emotion under normal and pathological conditions ; however , the interactions between them are essentially unknown .
	manualset3
165633	9	412492	7	NULL	NULL	0	NULL	 interactions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The serotonin system and NMDA receptors ( NMDARs ) in prefrontal cortex ( PFC ) are both critically involved in the regulation of cognition and emotion under normal and pathological conditions ; however , the interactions between them are essentially unknown .
	manualset3
165634	1	412493	7	NULL	NULL	0	NULL	classification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the classification by Dyck , this disorder could be referred to as hereditary motor and sensory neuropathy type V. Spastic paraplegia with amyotrophy is rare , but should be identified as a distinct disorder .
	manualset3
165635	2	412493	7	NULL	NULL	NULL	NULL	Dyck	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	According to the classification by Dyck , this disorder could be referred to as hereditary motor and sensory neuropathy type V. Spastic paraplegia with amyotrophy is rare , but should be identified as a distinct disorder .
	manualset3
165636	3	412493	7	NULL	NULL	0	NULL	disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the classification by Dyck , this disorder could be referred to as hereditary motor and sensory neuropathy type V. Spastic paraplegia with amyotrophy is rare , but should be identified as a distinct disorder .
	manualset3
165637	4	412493	7	NULL	NULL	0	NULL	hereditary motor type	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the classification by Dyck , this disorder could be referred to as hereditary motor and sensory neuropathy type V. Spastic paraplegia with amyotrophy is rare , but should be identified as a distinct disorder .
	manualset3
165638	5	412493	7	NULL	NULL	0	NULL	sensory neuropathy type	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the classification by Dyck , this disorder could be referred to as hereditary motor and sensory neuropathy type V. Spastic paraplegia with amyotrophy is rare , but should be identified as a distinct disorder .
	manualset3
165639	6	412493	7	NULL	NULL	0	NULL	V. Spastic paraplegia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the classification by Dyck , this disorder could be referred to as hereditary motor and sensory neuropathy type V. Spastic paraplegia with amyotrophy is rare , but should be identified as a distinct disorder .
	manualset3
165640	7	412493	7	NULL	NULL	0	NULL	amyotrophy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the classification by Dyck , this disorder could be referred to as hereditary motor and sensory neuropathy type V. Spastic paraplegia with amyotrophy is rare , but should be identified as a distinct disorder .
	manualset3
165641	8	412493	7	NULL	NULL	0	NULL	disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the classification by Dyck , this disorder could be referred to as hereditary motor and sensory neuropathy type V. Spastic paraplegia with amyotrophy is rare , but should be identified as a distinct disorder .
	manualset3
165642	1	412494	7	NULL	NULL	0	NULL	serum concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The serum concentrations of neuraminic acid , CEA , gamma-Gt , 5-nucleotidase , haptoglobin , and alkaline phosphatase were determined before therapy and three and six months after the initiation of therapy in 42 patients with small cell bronchial carcinomas .
	manualset3
165643	2	412494	7	NULL	NULL	0	NULL	neuraminic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The serum concentrations of neuraminic acid , CEA , gamma-Gt , 5-nucleotidase , haptoglobin , and alkaline phosphatase were determined before therapy and three and six months after the initiation of therapy in 42 patients with small cell bronchial carcinomas .
	manualset3
165644	3	412494	7	NULL	NULL	0	NULL	CEA	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The serum concentrations of neuraminic acid , CEA , gamma-Gt , 5-nucleotidase , haptoglobin , and alkaline phosphatase were determined before therapy and three and six months after the initiation of therapy in 42 patients with small cell bronchial carcinomas .
	manualset3
165645	4	412494	7	NULL	NULL	0	NULL	gamma-Gt , 5-nucleotidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The serum concentrations of neuraminic acid , CEA , gamma-Gt , 5-nucleotidase , haptoglobin , and alkaline phosphatase were determined before therapy and three and six months after the initiation of therapy in 42 patients with small cell bronchial carcinomas .
	manualset3
165646	5	412494	7	NULL	NULL	0	NULL	 haptoglobin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The serum concentrations of neuraminic acid , CEA , gamma-Gt , 5-nucleotidase , haptoglobin , and alkaline phosphatase were determined before therapy and three and six months after the initiation of therapy in 42 patients with small cell bronchial carcinomas .
	manualset3
165647	6	412494	7	NULL	NULL	0	NULL	alkaline phosphatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The serum concentrations of neuraminic acid , CEA , gamma-Gt , 5-nucleotidase , haptoglobin , and alkaline phosphatase were determined before therapy and three and six months after the initiation of therapy in 42 patients with small cell bronchial carcinomas .
	manualset3
165648	7	412494	7	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The serum concentrations of neuraminic acid , CEA , gamma-Gt , 5-nucleotidase , haptoglobin , and alkaline phosphatase were determined before therapy and three and six months after the initiation of therapy in 42 patients with small cell bronchial carcinomas .
	manualset3
165649	8	412494	7	NULL	NULL	0	NULL	 three months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The serum concentrations of neuraminic acid , CEA , gamma-Gt , 5-nucleotidase , haptoglobin , and alkaline phosphatase were determined before therapy and three and six months after the initiation of therapy in 42 patients with small cell bronchial carcinomas .
	manualset3
165650	9	412494	7	NULL	NULL	0	NULL	six months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The serum concentrations of neuraminic acid , CEA , gamma-Gt , 5-nucleotidase , haptoglobin , and alkaline phosphatase were determined before therapy and three and six months after the initiation of therapy in 42 patients with small cell bronchial carcinomas .
	manualset3
165651	10	412494	7	NULL	NULL	0	NULL	initiation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The serum concentrations of neuraminic acid , CEA , gamma-Gt , 5-nucleotidase , haptoglobin , and alkaline phosphatase were determined before therapy and three and six months after the initiation of therapy in 42 patients with small cell bronchial carcinomas .
	manualset3
165652	11	412494	7	NULL	NULL	0	NULL	 therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The serum concentrations of neuraminic acid , CEA , gamma-Gt , 5-nucleotidase , haptoglobin , and alkaline phosphatase were determined before therapy and three and six months after the initiation of therapy in 42 patients with small cell bronchial carcinomas .
	manualset3
165653	12	412494	7	NULL	NULL	0	NULL	42 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The serum concentrations of neuraminic acid , CEA , gamma-Gt , 5-nucleotidase , haptoglobin , and alkaline phosphatase were determined before therapy and three and six months after the initiation of therapy in 42 patients with small cell bronchial carcinomas .
	manualset3
165654	13	412494	7	NULL	NULL	0	NULL	small cell bronchial carcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The serum concentrations of neuraminic acid , CEA , gamma-Gt , 5-nucleotidase , haptoglobin , and alkaline phosphatase were determined before therapy and three and six months after the initiation of therapy in 42 patients with small cell bronchial carcinomas .
	manualset3
165655	1	412495	7	NULL	NULL	0	NULL	 serum levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The serum levels of aldosterone , corticosterone and prolactin increased significantly from 10 to 20 days , whereas those of arginine vasopressin were the same between 10 days and 20 days but increased significantly from 10 to 40 days .
	manualset3
165656	2	412495	7	NULL	NULL	0	NULL	aldosterone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The serum levels of aldosterone , corticosterone and prolactin increased significantly from 10 to 20 days , whereas those of arginine vasopressin were the same between 10 days and 20 days but increased significantly from 10 to 40 days .
	manualset3
165657	3	412495	7	NULL	NULL	0	NULL	 corticosterone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The serum levels of aldosterone , corticosterone and prolactin increased significantly from 10 to 20 days , whereas those of arginine vasopressin were the same between 10 days and 20 days but increased significantly from 10 to 40 days .
	manualset3
165658	4	412495	7	NULL	NULL	0	NULL	prolactin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The serum levels of aldosterone , corticosterone and prolactin increased significantly from 10 to 20 days , whereas those of arginine vasopressin were the same between 10 days and 20 days but increased significantly from 10 to 40 days .
	manualset3
165659	5	412495	7	NULL	NULL	0	NULL	10 to 20 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The serum levels of aldosterone , corticosterone and prolactin increased significantly from 10 to 20 days , whereas those of arginine vasopressin were the same between 10 days and 20 days but increased significantly from 10 to 40 days .
	manualset3
165660	6	412495	7	NULL	NULL	NULL	NULL	 arginine vasopressin	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The serum levels of aldosterone , corticosterone and prolactin increased significantly from 10 to 20 days , whereas those of arginine vasopressin were the same between 10 days and 20 days but increased significantly from 10 to 40 days .
	manualset3
165661	7	412495	7	NULL	NULL	0	NULL	10 days and 20 days 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The serum levels of aldosterone , corticosterone and prolactin increased significantly from 10 to 20 days , whereas those of arginine vasopressin were the same between 10 days and 20 days but increased significantly from 10 to 40 days .
	manualset3
165662	8	412495	7	NULL	NULL	0	NULL	10 to 40 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The serum levels of aldosterone , corticosterone and prolactin increased significantly from 10 to 20 days , whereas those of arginine vasopressin were the same between 10 days and 20 days but increased significantly from 10 to 40 days .
	manualset3
165663	1	412496	7	NULL	NULL	0	NULL	service	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The service is called the UltraClinics Process .
	manualset3
165664	2	412496	7	NULL	NULL	0	NULL	UltraClinics Process 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The service is called the UltraClinics Process .
	manualset3
165665	1	412497	7	NULL	NULL	0	NULL	 seven transmembrane protein Smoothened ( Smo )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The seven transmembrane protein Smoothened ( Smo ) is a critical component of the Hedgehog ( Hh ) signaling pathway and is regulated by phosphorylation , dimerization , and cell-surface accumulation upon Hh stimulation .
	manualset3
165666	2	412497	7	NULL	NULL	0	NULL	component	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The seven transmembrane protein Smoothened ( Smo ) is a critical component of the Hedgehog ( Hh ) signaling pathway and is regulated by phosphorylation , dimerization , and cell-surface accumulation upon Hh stimulation .
	manualset3
165667	3	412497	7	NULL	NULL	0	NULL	Hedgehog ( Hh ) signaling pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The seven transmembrane protein Smoothened ( Smo ) is a critical component of the Hedgehog ( Hh ) signaling pathway and is regulated by phosphorylation , dimerization , and cell-surface accumulation upon Hh stimulation .
	manualset3
165668	4	412497	7	NULL	NULL	0	NULL	phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The seven transmembrane protein Smoothened ( Smo ) is a critical component of the Hedgehog ( Hh ) signaling pathway and is regulated by phosphorylation , dimerization , and cell-surface accumulation upon Hh stimulation .
	manualset3
165669	5	412497	7	NULL	NULL	0	NULL	dimerization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The seven transmembrane protein Smoothened ( Smo ) is a critical component of the Hedgehog ( Hh ) signaling pathway and is regulated by phosphorylation , dimerization , and cell-surface accumulation upon Hh stimulation .
	manualset3
165670	6	412497	7	NULL	NULL	0	NULL	cell-surface accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The seven transmembrane protein Smoothened ( Smo ) is a critical component of the Hedgehog ( Hh ) signaling pathway and is regulated by phosphorylation , dimerization , and cell-surface accumulation upon Hh stimulation .
	manualset3
165671	7	412497	7	NULL	NULL	0	NULL	Hh stimulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The seven transmembrane protein Smoothened ( Smo ) is a critical component of the Hedgehog ( Hh ) signaling pathway and is regulated by phosphorylation , dimerization , and cell-surface accumulation upon Hh stimulation .
	manualset3
165672	1	412498	7	NULL	NULL	0	NULL	 severe hyperinfection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The severe hyperinfection strongly suggested autoinfection , probably associated with depressed immunologic competence due to chronic stress .
	manualset3
165673	2	412498	7	NULL	NULL	0	NULL	autoinfection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The severe hyperinfection strongly suggested autoinfection , probably associated with depressed immunologic competence due to chronic stress .
	manualset3
165674	3	412498	7	NULL	NULL	0	NULL	immunologic competence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The severe hyperinfection strongly suggested autoinfection , probably associated with depressed immunologic competence due to chronic stress .
	manualset3
165675	4	412498	7	NULL	NULL	0	NULL	chronic stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The severe hyperinfection strongly suggested autoinfection , probably associated with depressed immunologic competence due to chronic stress .
	manualset3
165676	1	412499	7	NULL	NULL	0	NULL	severe hypoxemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The severe hypoxemia and modest anaerobic metabolism in association with marked tachypnea and normocapnia are consistent with small airway obstruction and wasted ventilation , since no change in arterial blood pressure , heart rate , hematocrit , hemoglobin , or blood volume was noted .
	manualset3
165677	2	412499	7	NULL	NULL	0	NULL	modest anaerobic metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The severe hypoxemia and modest anaerobic metabolism in association with marked tachypnea and normocapnia are consistent with small airway obstruction and wasted ventilation , since no change in arterial blood pressure , heart rate , hematocrit , hemoglobin , or blood volume was noted .
	manualset3
165678	3	412499	7	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The severe hypoxemia and modest anaerobic metabolism in association with marked tachypnea and normocapnia are consistent with small airway obstruction and wasted ventilation , since no change in arterial blood pressure , heart rate , hematocrit , hemoglobin , or blood volume was noted .
	manualset3
165679	4	412499	7	NULL	NULL	0	NULL	marked tachypnea	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The severe hypoxemia and modest anaerobic metabolism in association with marked tachypnea and normocapnia are consistent with small airway obstruction and wasted ventilation , since no change in arterial blood pressure , heart rate , hematocrit , hemoglobin , or blood volume was noted .
	manualset3
165680	5	412499	7	NULL	NULL	0	NULL	normocapnia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The severe hypoxemia and modest anaerobic metabolism in association with marked tachypnea and normocapnia are consistent with small airway obstruction and wasted ventilation , since no change in arterial blood pressure , heart rate , hematocrit , hemoglobin , or blood volume was noted .
	manualset3
165681	6	412499	7	NULL	NULL	0	NULL	small airway obstruction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The severe hypoxemia and modest anaerobic metabolism in association with marked tachypnea and normocapnia are consistent with small airway obstruction and wasted ventilation , since no change in arterial blood pressure , heart rate , hematocrit , hemoglobin , or blood volume was noted .
	manualset3
165682	7	412499	7	NULL	NULL	0	NULL	wasted ventilation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The severe hypoxemia and modest anaerobic metabolism in association with marked tachypnea and normocapnia are consistent with small airway obstruction and wasted ventilation , since no change in arterial blood pressure , heart rate , hematocrit , hemoglobin , or blood volume was noted .
	manualset3
165683	8	412499	7	NULL	NULL	0	NULL	arterial blood pressure	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The severe hypoxemia and modest anaerobic metabolism in association with marked tachypnea and normocapnia are consistent with small airway obstruction and wasted ventilation , since no change in arterial blood pressure , heart rate , hematocrit , hemoglobin , or blood volume was noted .
	manualset3
165684	9	412499	7	NULL	NULL	0	NULL	heart rate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The severe hypoxemia and modest anaerobic metabolism in association with marked tachypnea and normocapnia are consistent with small airway obstruction and wasted ventilation , since no change in arterial blood pressure , heart rate , hematocrit , hemoglobin , or blood volume was noted .
	manualset3
165685	10	412499	7	NULL	NULL	0	NULL	hematocrit	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The severe hypoxemia and modest anaerobic metabolism in association with marked tachypnea and normocapnia are consistent with small airway obstruction and wasted ventilation , since no change in arterial blood pressure , heart rate , hematocrit , hemoglobin , or blood volume was noted .
	manualset3
165686	11	412499	7	NULL	NULL	0	NULL	hemoglobin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The severe hypoxemia and modest anaerobic metabolism in association with marked tachypnea and normocapnia are consistent with small airway obstruction and wasted ventilation , since no change in arterial blood pressure , heart rate , hematocrit , hemoglobin , or blood volume was noted .
	manualset3
165687	12	412499	7	NULL	NULL	0	NULL	blood volume 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The severe hypoxemia and modest anaerobic metabolism in association with marked tachypnea and normocapnia are consistent with small airway obstruction and wasted ventilation , since no change in arterial blood pressure , heart rate , hematocrit , hemoglobin , or blood volume was noted .
	manualset3
165688	1	412500	7	NULL	NULL	0	NULL	severity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The severity and extent of infection in peripheral tissues peaked at day 1 PI .
	manualset3
165689	2	412500	7	NULL	NULL	0	NULL	extent	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The severity and extent of infection in peripheral tissues peaked at day 1 PI .
	manualset3
165690	3	412500	7	NULL	NULL	0	NULL	 infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The severity and extent of infection in peripheral tissues peaked at day 1 PI .
	manualset3
165691	4	412500	7	NULL	NULL	0	NULL	 peripheral tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The severity and extent of infection in peripheral tissues peaked at day 1 PI .
	manualset3
165692	5	412500	7	NULL	NULL	0	NULL	day 1	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The severity and extent of infection in peripheral tissues peaked at day 1 PI .
	manualset3
165693	6	412500	7	NULL	NULL	0	NULL	PI	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The severity and extent of infection in peripheral tissues peaked at day 1 PI .
	manualset3
165694	1	412501	7	NULL	NULL	0	NULL	 severity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The severity of OSA was determined from the apnea - hypopnea index ( AHI ) for total sleep time ( AHI ( TST ) ) , and was classified as mild ( 5 to 25 events/h ) , moderate ( 26 to 50 events/h ) , and severe ( ) 50/events/h ) .
	manualset3
165695	2	412501	7	NULL	NULL	NULL	NULL	OSA	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The severity of OSA was determined from the apnea - hypopnea index ( AHI ) for total sleep time ( AHI ( TST ) ) , and was classified as mild ( 5 to 25 events/h ) , moderate ( 26 to 50 events/h ) , and severe ( ) 50/events/h ) .
	manualset3
165696	3	412501	7	NULL	NULL	0	NULL	apnea - hypopnea index ( AHI )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The severity of OSA was determined from the apnea - hypopnea index ( AHI ) for total sleep time ( AHI ( TST ) ) , and was classified as mild ( 5 to 25 events/h ) , moderate ( 26 to 50 events/h ) , and severe ( ) 50/events/h ) .
	manualset3
165697	4	412501	7	NULL	NULL	0	NULL	total sleep time ( AHI ( TST ) )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The severity of OSA was determined from the apnea - hypopnea index ( AHI ) for total sleep time ( AHI ( TST ) ) , and was classified as mild ( 5 to 25 events/h ) , moderate ( 26 to 50 events/h ) , and severe ( ) 50/events/h ) .
	manualset3
165699	6	412501	7	NULL	NULL	0	NULL	5 to 25 events/h	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The severity of OSA was determined from the apnea - hypopnea index ( AHI ) for total sleep time ( AHI ( TST ) ) , and was classified as mild ( 5 to 25 events/h ) , moderate ( 26 to 50 events/h ) , and severe ( ) 50/events/h ) .
	manualset3
165701	8	412501	7	NULL	NULL	0	NULL	26 to 50 events/h 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The severity of OSA was determined from the apnea - hypopnea index ( AHI ) for total sleep time ( AHI ( TST ) ) , and was classified as mild ( 5 to 25 events/h ) , moderate ( 26 to 50 events/h ) , and severe ( ) 50/events/h ) .
	manualset3
165703	10	412501	7	NULL	NULL	0	NULL	50/events/h	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The severity of OSA was determined from the apnea - hypopnea index ( AHI ) for total sleep time ( AHI ( TST ) ) , and was classified as mild ( 5 to 25 events/h ) , moderate ( 26 to 50 events/h ) , and severe ( ) 50/events/h ) .
	manualset3
165704	1	412502	7	NULL	NULL	0	NULL	Clinico-morphocytochemical 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinico-morphocytochemical parallels in different courses of chronic lympholeukemia ) .
	manualset3
165705	2	412502	7	NULL	NULL	0	NULL	 courses	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinico-morphocytochemical parallels in different courses of chronic lympholeukemia ) .
	manualset3
165706	3	412502	7	NULL	NULL	0	NULL	chronic lympholeukemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinico-morphocytochemical parallels in different courses of chronic lympholeukemia ) .
	manualset3
165707	1	412503	7	NULL	NULL	0	NULL	severity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The severity of the experimental colitis was shown to be directly related to the concentration of the detergent .
	manualset3
165708	2	412503	7	NULL	NULL	0	NULL	experimental colitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The severity of the experimental colitis was shown to be directly related to the concentration of the detergent .
	manualset3
165709	3	412503	7	NULL	NULL	0	NULL	concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The severity of the experimental colitis was shown to be directly related to the concentration of the detergent .
	manualset3
165710	4	412503	7	NULL	NULL	0	NULL	detergent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The severity of the experimental colitis was shown to be directly related to the concentration of the detergent .
	manualset3
165711	1	412504	7	NULL	NULL	0	NULL	sexual abuse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The sexual abuse and rape of young girls , pregnancy during adolescent years , and abandonment of women to raise or support children are , overwhelmingly , adult male behavior problems exacerbated by poverty .
	manualset3
165712	2	412504	7	NULL	NULL	0	NULL	 rape 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The sexual abuse and rape of young girls , pregnancy during adolescent years , and abandonment of women to raise or support children are , overwhelmingly , adult male behavior problems exacerbated by poverty .
	manualset3
165713	3	412504	7	NULL	NULL	0	NULL	young girls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The sexual abuse and rape of young girls , pregnancy during adolescent years , and abandonment of women to raise or support children are , overwhelmingly , adult male behavior problems exacerbated by poverty .
	manualset3
165714	4	412504	7	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The sexual abuse and rape of young girls , pregnancy during adolescent years , and abandonment of women to raise or support children are , overwhelmingly , adult male behavior problems exacerbated by poverty .
	manualset3
165715	5	412504	7	NULL	NULL	0	NULL	adolescent years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The sexual abuse and rape of young girls , pregnancy during adolescent years , and abandonment of women to raise or support children are , overwhelmingly , adult male behavior problems exacerbated by poverty .
	manualset3
165716	6	412504	7	NULL	NULL	0	NULL	abandonment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The sexual abuse and rape of young girls , pregnancy during adolescent years , and abandonment of women to raise or support children are , overwhelmingly , adult male behavior problems exacerbated by poverty .
	manualset3
165717	7	412504	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The sexual abuse and rape of young girls , pregnancy during adolescent years , and abandonment of women to raise or support children are , overwhelmingly , adult male behavior problems exacerbated by poverty .
	manualset3
165718	8	412504	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The sexual abuse and rape of young girls , pregnancy during adolescent years , and abandonment of women to raise or support children are , overwhelmingly , adult male behavior problems exacerbated by poverty .
	manualset3
165719	9	412504	7	NULL	NULL	0	NULL	adult male behavior problems 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The sexual abuse and rape of young girls , pregnancy during adolescent years , and abandonment of women to raise or support children are , overwhelmingly , adult male behavior problems exacerbated by poverty .
	manualset3
165720	10	412504	7	NULL	NULL	0	NULL	 poverty	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The sexual abuse and rape of young girls , pregnancy during adolescent years , and abandonment of women to raise or support children are , overwhelmingly , adult male behavior problems exacerbated by poverty .
	manualset3
165721	1	412505	7	NULL	NULL	0	NULL	sham-operated mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The sham-operated mice were fed the control diet and OVX mice were fed diets containing genistein or Novasoy or the control diet , with or without 17beta-estradiol treatment , for 5 wk .
	manualset3
165722	2	412505	7	NULL	NULL	0	NULL	control diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The sham-operated mice were fed the control diet and OVX mice were fed diets containing genistein or Novasoy or the control diet , with or without 17beta-estradiol treatment , for 5 wk .
	manualset3
165723	3	412505	7	NULL	NULL	0	NULL	OVX mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The sham-operated mice were fed the control diet and OVX mice were fed diets containing genistein or Novasoy or the control diet , with or without 17beta-estradiol treatment , for 5 wk .
	manualset3
165724	4	412505	7	NULL	NULL	NULL	NULL	genistein	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The sham-operated mice were fed the control diet and OVX mice were fed diets containing genistein or Novasoy or the control diet , with or without 17beta-estradiol treatment , for 5 wk .
	manualset3
165725	5	412505	7	NULL	NULL	NULL	NULL	Novasoy	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The sham-operated mice were fed the control diet and OVX mice were fed diets containing genistein or Novasoy or the control diet , with or without 17beta-estradiol treatment , for 5 wk .
	manualset3
165726	6	412505	7	NULL	NULL	0	NULL	control diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The sham-operated mice were fed the control diet and OVX mice were fed diets containing genistein or Novasoy or the control diet , with or without 17beta-estradiol treatment , for 5 wk .
	manualset3
165727	7	412505	7	NULL	NULL	0	NULL	17beta-estradiol treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The sham-operated mice were fed the control diet and OVX mice were fed diets containing genistein or Novasoy or the control diet , with or without 17beta-estradiol treatment , for 5 wk .
	manualset3
165728	8	412505	7	NULL	NULL	0	NULL	5 wk	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The sham-operated mice were fed the control diet and OVX mice were fed diets containing genistein or Novasoy or the control diet , with or without 17beta-estradiol treatment , for 5 wk .
	manualset3
166505	9	412505	7	NULL	NULL	0	NULL	diets	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The sham-operated mice were fed the control diet and OVX mice were fed diets containing genistein or Novasoy or the control diet , with or without 17beta-estradiol treatment , for 5 wk .
	manualset3
165729	1	412506	7	NULL	NULL	0	NULL	shape 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The shape and morphology of the particles was studied using electron microscopy .
	manualset3
165730	2	412506	7	NULL	NULL	0	NULL	morphology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The shape and morphology of the particles was studied using electron microscopy .
	manualset3
165731	3	412506	7	NULL	NULL	0	NULL	 particles	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The shape and morphology of the particles was studied using electron microscopy .
	manualset3
165732	4	412506	7	NULL	NULL	0	NULL	electron microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The shape and morphology of the particles was studied using electron microscopy .
	manualset3
165733	1	412507	7	NULL	NULL	0	NULL	shifts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The shifts are attributed to the phenyl moiety in the 4-ferrocene thiophenol and dielectric constant of the solvation environment .
	manualset3
165734	2	412507	7	NULL	NULL	0	NULL	phenyl moiety	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The shifts are attributed to the phenyl moiety in the 4-ferrocene thiophenol and dielectric constant of the solvation environment .
	manualset3
165735	3	412507	7	NULL	NULL	0	NULL	4-ferrocene thiophenol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The shifts are attributed to the phenyl moiety in the 4-ferrocene thiophenol and dielectric constant of the solvation environment .
	manualset3
165736	4	412507	7	NULL	NULL	0	NULL	dielectric constant	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The shifts are attributed to the phenyl moiety in the 4-ferrocene thiophenol and dielectric constant of the solvation environment .
	manualset3
165737	5	412507	7	NULL	NULL	0	NULL	solvation environment	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The shifts are attributed to the phenyl moiety in the 4-ferrocene thiophenol and dielectric constant of the solvation environment .
	manualset3
165738	1	412508	7	NULL	NULL	NULL	NULL	short-form version	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The short-form version of the Depression Anxiety Stress Scales ( DASS-21 ) : construct validity and normative data in a large non-clinical sample .
	manualset3
165739	2	412508	7	NULL	NULL	NULL	NULL	Depression Anxiety Stress Scales ( DASS-21 )	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The short-form version of the Depression Anxiety Stress Scales ( DASS-21 ) : construct validity and normative data in a large non-clinical sample .
	manualset3
165740	3	412508	7	NULL	NULL	0	NULL	normative data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The short-form version of the Depression Anxiety Stress Scales ( DASS-21 ) : construct validity and normative data in a large non-clinical sample .
	manualset3
165741	4	412508	7	NULL	NULL	NULL	NULL	non-clinical sample 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The short-form version of the Depression Anxiety Stress Scales ( DASS-21 ) : construct validity and normative data in a large non-clinical sample .
	manualset3
166506	5	412508	7	NULL	NULL	0	NULL	validity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The short-form version of the Depression Anxiety Stress Scales ( DASS-21 ) : construct validity and normative data in a large non-clinical sample .
	manualset3
165742	1	412509	7	NULL	NULL	NULL	NULL	shortage	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The shortage of good quality water resources is becoming an important issue in arid and semi-arid zones .
	manualset3
165743	2	412509	7	NULL	NULL	0	NULL	 water resources	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The shortage of good quality water resources is becoming an important issue in arid and semi-arid zones .
	manualset3
165744	3	412509	7	NULL	NULL	0	NULL	issue	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The shortage of good quality water resources is becoming an important issue in arid and semi-arid zones .
	manualset3
165745	4	412509	7	NULL	NULL	0	NULL	 arid zones	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The shortage of good quality water resources is becoming an important issue in arid and semi-arid zones .
	manualset3
165746	5	412509	7	NULL	NULL	0	NULL	semi-arid zones	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The shortage of good quality water resources is becoming an important issue in arid and semi-arid zones .
	manualset3
166507	6	412509	7	NULL	NULL	0	NULL	quality	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The shortage of good quality water resources is becoming an important issue in arid and semi-arid zones .
	manualset3
165747	1	412510	7	NULL	NULL	0	NULL	sialated , presumed-globular form of an atypical pseudocholinesterase ( pseudo-ChE )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The sialated , presumed-globular form of an atypical pseudocholinesterase ( pseudo-ChE ) previously described from surgeonfish tissues ( Leibel : Comparative Biochemistry and Physiology 1988 ) has been purified to apparent homogeneity using a combination of salt fractionation along with ion-exchange and concanavalin A-Sepharose affinity chromatographic techniques .
	manualset3
165748	2	412510	7	NULL	NULL	0	NULL	surgeonfish tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The sialated , presumed-globular form of an atypical pseudocholinesterase ( pseudo-ChE ) previously described from surgeonfish tissues ( Leibel : Comparative Biochemistry and Physiology 1988 ) has been purified to apparent homogeneity using a combination of salt fractionation along with ion-exchange and concanavalin A-Sepharose affinity chromatographic techniques .
	manualset3
165749	3	412510	7	NULL	NULL	0	NULL	Leibel	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	The sialated , presumed-globular form of an atypical pseudocholinesterase ( pseudo-ChE ) previously described from surgeonfish tissues ( Leibel : Comparative Biochemistry and Physiology 1988 ) has been purified to apparent homogeneity using a combination of salt fractionation along with ion-exchange and concanavalin A-Sepharose affinity chromatographic techniques .
	manualset3
165750	4	412510	7	NULL	NULL	0	NULL	Comparative Biochemistry and Physiology	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	The sialated , presumed-globular form of an atypical pseudocholinesterase ( pseudo-ChE ) previously described from surgeonfish tissues ( Leibel : Comparative Biochemistry and Physiology 1988 ) has been purified to apparent homogeneity using a combination of salt fractionation along with ion-exchange and concanavalin A-Sepharose affinity chromatographic techniques .
	manualset3
165751	5	412510	7	NULL	NULL	0	NULL	1988 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The sialated , presumed-globular form of an atypical pseudocholinesterase ( pseudo-ChE ) previously described from surgeonfish tissues ( Leibel : Comparative Biochemistry and Physiology 1988 ) has been purified to apparent homogeneity using a combination of salt fractionation along with ion-exchange and concanavalin A-Sepharose affinity chromatographic techniques .
	manualset3
165752	6	412510	7	NULL	NULL	0	NULL	homogeneity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The sialated , presumed-globular form of an atypical pseudocholinesterase ( pseudo-ChE ) previously described from surgeonfish tissues ( Leibel : Comparative Biochemistry and Physiology 1988 ) has been purified to apparent homogeneity using a combination of salt fractionation along with ion-exchange and concanavalin A-Sepharose affinity chromatographic techniques .
	manualset3
165753	7	412510	7	NULL	NULL	0	NULL	salt fractionation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The sialated , presumed-globular form of an atypical pseudocholinesterase ( pseudo-ChE ) previously described from surgeonfish tissues ( Leibel : Comparative Biochemistry and Physiology 1988 ) has been purified to apparent homogeneity using a combination of salt fractionation along with ion-exchange and concanavalin A-Sepharose affinity chromatographic techniques .
	manualset3
165754	8	412510	7	NULL	NULL	0	NULL	ion-exchange 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The sialated , presumed-globular form of an atypical pseudocholinesterase ( pseudo-ChE ) previously described from surgeonfish tissues ( Leibel : Comparative Biochemistry and Physiology 1988 ) has been purified to apparent homogeneity using a combination of salt fractionation along with ion-exchange and concanavalin A-Sepharose affinity chromatographic techniques .
	manualset3
165755	9	412510	7	NULL	NULL	0	NULL	concanavalin A-Sepharose affinity chromatographic techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The sialated , presumed-globular form of an atypical pseudocholinesterase ( pseudo-ChE ) previously described from surgeonfish tissues ( Leibel : Comparative Biochemistry and Physiology 1988 ) has been purified to apparent homogeneity using a combination of salt fractionation along with ion-exchange and concanavalin A-Sepharose affinity chromatographic techniques .
	manualset3
173645	10	412510	7	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The sialated , presumed-globular form of an atypical pseudocholinesterase ( pseudo-ChE ) previously described from surgeonfish tissues ( Leibel : Comparative Biochemistry and Physiology 1988 ) has been purified to apparent homogeneity using a combination of salt fractionation along with ion-exchange and concanavalin A-Sepharose affinity chromatographic techniques .
	manualset3
165756	1	412511	7	NULL	NULL	0	NULL	sialidase gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The sialidase gene was detected on two restriction fragments ( HincII , HindIII ) of chromosomal DNA and their correct recombination resulted in an active enzyme expressed by Escherichia coli .
	manualset3
165757	2	412511	7	NULL	NULL	0	NULL	two restriction fragments ( HincII , HindIII )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The sialidase gene was detected on two restriction fragments ( HincII , HindIII ) of chromosomal DNA and their correct recombination resulted in an active enzyme expressed by Escherichia coli .
	manualset3
165758	3	412511	7	NULL	NULL	0	NULL	chromosomal DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The sialidase gene was detected on two restriction fragments ( HincII , HindIII ) of chromosomal DNA and their correct recombination resulted in an active enzyme expressed by Escherichia coli .
	manualset3
165759	4	412511	7	NULL	NULL	0	NULL	recombination	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The sialidase gene was detected on two restriction fragments ( HincII , HindIII ) of chromosomal DNA and their correct recombination resulted in an active enzyme expressed by Escherichia coli .
	manualset3
165760	5	412511	7	NULL	NULL	0	NULL	active enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The sialidase gene was detected on two restriction fragments ( HincII , HindIII ) of chromosomal DNA and their correct recombination resulted in an active enzyme expressed by Escherichia coli .
	manualset3
165761	6	412511	7	NULL	NULL	0	NULL	Escherichia coli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The sialidase gene was detected on two restriction fragments ( HincII , HindIII ) of chromosomal DNA and their correct recombination resulted in an active enzyme expressed by Escherichia coli .
	manualset3
165762	1	412512	7	NULL	NULL	0	NULL	 literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the literature , intracranial metastasis of a bronchogenic carcinoma bleeds more often than that of other carcinomas .
	manualset3
165763	2	412512	7	NULL	NULL	0	NULL	 intracranial metastasis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the literature , intracranial metastasis of a bronchogenic carcinoma bleeds more often than that of other carcinomas .
	manualset3
165764	3	412512	7	NULL	NULL	NULL	NULL	bronchogenic carcinoma 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	According to the literature , intracranial metastasis of a bronchogenic carcinoma bleeds more often than that of other carcinomas .
	manualset3
165765	4	412512	7	NULL	NULL	0	NULL	carcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the literature , intracranial metastasis of a bronchogenic carcinoma bleeds more often than that of other carcinomas .
	manualset3
165766	1	412513	7	NULL	NULL	0	NULL	side effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The side effects associated with prostaglandin use include nausea , vomiting , diarrhea , heat waves , shivering , headache , dizziness , elevated temperatures , and leucocytosis .
	manualset3
165767	2	412513	7	NULL	NULL	0	NULL	prostaglandin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The side effects associated with prostaglandin use include nausea , vomiting , diarrhea , heat waves , shivering , headache , dizziness , elevated temperatures , and leucocytosis .
	manualset3
165768	3	412513	7	NULL	NULL	0	NULL	nausea	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The side effects associated with prostaglandin use include nausea , vomiting , diarrhea , heat waves , shivering , headache , dizziness , elevated temperatures , and leucocytosis .
	manualset3
165769	4	412513	7	NULL	NULL	0	NULL	vomiting	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The side effects associated with prostaglandin use include nausea , vomiting , diarrhea , heat waves , shivering , headache , dizziness , elevated temperatures , and leucocytosis .
	manualset3
165770	5	412513	7	NULL	NULL	0	NULL	diarrhea	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The side effects associated with prostaglandin use include nausea , vomiting , diarrhea , heat waves , shivering , headache , dizziness , elevated temperatures , and leucocytosis .
	manualset3
165771	6	412513	7	NULL	NULL	0	NULL	heat waves	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The side effects associated with prostaglandin use include nausea , vomiting , diarrhea , heat waves , shivering , headache , dizziness , elevated temperatures , and leucocytosis .
	manualset3
165772	7	412513	7	NULL	NULL	0	NULL	shivering	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The side effects associated with prostaglandin use include nausea , vomiting , diarrhea , heat waves , shivering , headache , dizziness , elevated temperatures , and leucocytosis .
	manualset3
165773	8	412513	7	NULL	NULL	0	NULL	headache	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The side effects associated with prostaglandin use include nausea , vomiting , diarrhea , heat waves , shivering , headache , dizziness , elevated temperatures , and leucocytosis .
	manualset3
165774	9	412513	7	NULL	NULL	0	NULL	dizziness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The side effects associated with prostaglandin use include nausea , vomiting , diarrhea , heat waves , shivering , headache , dizziness , elevated temperatures , and leucocytosis .
	manualset3
165775	10	412513	7	NULL	NULL	0	NULL	 elevated temperatures 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The side effects associated with prostaglandin use include nausea , vomiting , diarrhea , heat waves , shivering , headache , dizziness , elevated temperatures , and leucocytosis .
	manualset3
165776	11	412513	7	NULL	NULL	0	NULL	leucocytosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The side effects associated with prostaglandin use include nausea , vomiting , diarrhea , heat waves , shivering , headache , dizziness , elevated temperatures , and leucocytosis .
	manualset3
165777	1	412514	7	NULL	NULL	0	NULL	signal transduction pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The signal transduction pathways involved in the regulation of the acrosome reaction and motility of fowl spermatozoa were investigated .
	manualset3
165778	2	412514	7	NULL	NULL	0	NULL	regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The signal transduction pathways involved in the regulation of the acrosome reaction and motility of fowl spermatozoa were investigated .
	manualset3
165779	3	412514	7	NULL	NULL	0	NULL	acrosome reaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The signal transduction pathways involved in the regulation of the acrosome reaction and motility of fowl spermatozoa were investigated .
	manualset3
165780	4	412514	7	NULL	NULL	0	NULL	motility	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The signal transduction pathways involved in the regulation of the acrosome reaction and motility of fowl spermatozoa were investigated .
	manualset3
165781	5	412514	7	NULL	NULL	0	NULL	fowl spermatozoa	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The signal transduction pathways involved in the regulation of the acrosome reaction and motility of fowl spermatozoa were investigated .
	manualset3
165782	1	412515	7	NULL	NULL	0	NULL	signal transduction pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The signal transduction pathways responsible for cell cycle activation by CSb-9 include Gi-mediated activation of extracellular signal-regulated kinase 1 and phosphatidylinositol 3-kinase ( PI3-K ) .
	manualset3
165783	2	412515	7	NULL	NULL	0	NULL	cell cycle activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The signal transduction pathways responsible for cell cycle activation by CSb-9 include Gi-mediated activation of extracellular signal-regulated kinase 1 and phosphatidylinositol 3-kinase ( PI3-K ) .
	manualset3
165784	3	412515	7	NULL	NULL	0	NULL	 CSb-9	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The signal transduction pathways responsible for cell cycle activation by CSb-9 include Gi-mediated activation of extracellular signal-regulated kinase 1 and phosphatidylinositol 3-kinase ( PI3-K ) .
	manualset3
165785	4	412515	7	NULL	NULL	0	NULL	Gi-mediated activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The signal transduction pathways responsible for cell cycle activation by CSb-9 include Gi-mediated activation of extracellular signal-regulated kinase 1 and phosphatidylinositol 3-kinase ( PI3-K ) .
	manualset3
165786	5	412515	7	NULL	NULL	0	NULL	extracellular signal-regulated kinase 1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The signal transduction pathways responsible for cell cycle activation by CSb-9 include Gi-mediated activation of extracellular signal-regulated kinase 1 and phosphatidylinositol 3-kinase ( PI3-K ) .
	manualset3
165787	6	412515	7	NULL	NULL	0	NULL	phosphatidylinositol 3-kinase ( PI3-K )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The signal transduction pathways responsible for cell cycle activation by CSb-9 include Gi-mediated activation of extracellular signal-regulated kinase 1 and phosphatidylinositol 3-kinase ( PI3-K ) .
	manualset3
165788	1	412516	7	NULL	NULL	0	NULL	 signaling pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The signaling pathways underlying egress have been characterized through the use of pharmacological agents acting on different aspects of the pathways .
	manualset3
165789	2	412516	7	NULL	NULL	NULL	NULL	egress	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The signaling pathways underlying egress have been characterized through the use of pharmacological agents acting on different aspects of the pathways .
	manualset3
165790	3	412516	7	NULL	NULL	NULL	NULL	pharmacological agents	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The signaling pathways underlying egress have been characterized through the use of pharmacological agents acting on different aspects of the pathways .
	manualset3
165791	4	412516	7	NULL	NULL	0	NULL	aspects 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The signaling pathways underlying egress have been characterized through the use of pharmacological agents acting on different aspects of the pathways .
	manualset3
165792	5	412516	7	NULL	NULL	0	NULL	pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The signaling pathways underlying egress have been characterized through the use of pharmacological agents acting on different aspects of the pathways .
	manualset3
165793	1	412517	7	NULL	NULL	0	NULL	signals	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The signals are blocked by mucosal amiloride in low microM concentrations .
	manualset3
165794	2	412517	7	NULL	NULL	0	NULL	mucosal amiloride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The signals are blocked by mucosal amiloride in low microM concentrations .
	manualset3
165795	3	412517	7	NULL	NULL	0	NULL	low microM concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The signals are blocked by mucosal amiloride in low microM concentrations .
	manualset3
165796	1	412518	7	NULL	NULL	0	NULL	bone scan abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The significance of bone scan abnormalities in patients with primary osteogenic sarcoma .
	manualset3
165797	2	412518	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The significance of bone scan abnormalities in patients with primary osteogenic sarcoma .
	manualset3
165798	3	412518	7	NULL	NULL	0	NULL	primary osteogenic sarcoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The significance of bone scan abnormalities in patients with primary osteogenic sarcoma .
	manualset3
165799	1	412519	7	NULL	NULL	0	NULL	phase I introns	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The significance of the predominance of phase I introns , the almost uniformly short length of the 42 introns and the overall small size of the gene , is discussed in relation to the evolution of multifunctional proteins .
	manualset3
165800	2	412519	7	NULL	NULL	0	NULL	short length	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The significance of the predominance of phase I introns , the almost uniformly short length of the 42 introns and the overall small size of the gene , is discussed in relation to the evolution of multifunctional proteins .
	manualset3
165801	3	412519	7	NULL	NULL	0	NULL	42 introns	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The significance of the predominance of phase I introns , the almost uniformly short length of the 42 introns and the overall small size of the gene , is discussed in relation to the evolution of multifunctional proteins .
	manualset3
165802	4	412519	7	NULL	NULL	0	NULL	small size 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The significance of the predominance of phase I introns , the almost uniformly short length of the 42 introns and the overall small size of the gene , is discussed in relation to the evolution of multifunctional proteins .
	manualset3
165803	5	412519	7	NULL	NULL	0	NULL	gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The significance of the predominance of phase I introns , the almost uniformly short length of the 42 introns and the overall small size of the gene , is discussed in relation to the evolution of multifunctional proteins .
	manualset3
165804	6	412519	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The significance of the predominance of phase I introns , the almost uniformly short length of the 42 introns and the overall small size of the gene , is discussed in relation to the evolution of multifunctional proteins .
	manualset3
165805	7	412519	7	NULL	NULL	0	NULL	 evolution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The significance of the predominance of phase I introns , the almost uniformly short length of the 42 introns and the overall small size of the gene , is discussed in relation to the evolution of multifunctional proteins .
	manualset3
165806	8	412519	7	NULL	NULL	0	NULL	multifunctional proteins	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The significance of the predominance of phase I introns , the almost uniformly short length of the 42 introns and the overall small size of the gene , is discussed in relation to the evolution of multifunctional proteins .
	manualset3
173646	9	412519	7	NULL	NULL	0	NULL	significance	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The significance of the predominance of phase I introns , the almost uniformly short length of the 42 introns and the overall small size of the gene , is discussed in relation to the evolution of multifunctional proteins .
	manualset3
165807	1	412520	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the patient , this lesion had a progressive and slow growth of about two years .
	manualset3
165808	2	412520	7	NULL	NULL	0	NULL	lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the patient , this lesion had a progressive and slow growth of about two years .
	manualset3
165809	3	412520	7	NULL	NULL	0	NULL	slow growth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the patient , this lesion had a progressive and slow growth of about two years .
	manualset3
165810	4	412520	7	NULL	NULL	0	NULL	two years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the patient , this lesion had a progressive and slow growth of about two years .
	manualset3
165811	1	412521	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The significance of the studies on the forestomach and bladder epithelia are discussed .
	manualset3
165812	2	412521	7	NULL	NULL	0	NULL	forestomach	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The significance of the studies on the forestomach and bladder epithelia are discussed .
	manualset3
165813	3	412521	7	NULL	NULL	0	NULL	bladder epithelia	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The significance of the studies on the forestomach and bladder epithelia are discussed .
	manualset3
165814	1	412522	7	NULL	NULL	NULL	NULL	decrease	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The significant decrease in II-hydroxycorticosteroids ( II-OCS ) , adrenaline , noradrenaline , dopamine , and a tendency to the increase in histamine content were observed in the venous blood plasma .
	manualset3
165815	2	412522	7	NULL	NULL	0	NULL	II-hydroxycorticosteroids ( II-OCS )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The significant decrease in II-hydroxycorticosteroids ( II-OCS ) , adrenaline , noradrenaline , dopamine , and a tendency to the increase in histamine content were observed in the venous blood plasma .
	manualset3
165816	3	412522	7	NULL	NULL	0	NULL	adrenaline	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The significant decrease in II-hydroxycorticosteroids ( II-OCS ) , adrenaline , noradrenaline , dopamine , and a tendency to the increase in histamine content were observed in the venous blood plasma .
	manualset3
165817	4	412522	7	NULL	NULL	0	NULL	noradrenaline	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The significant decrease in II-hydroxycorticosteroids ( II-OCS ) , adrenaline , noradrenaline , dopamine , and a tendency to the increase in histamine content were observed in the venous blood plasma .
	manualset3
165818	5	412522	7	NULL	NULL	0	NULL	dopamine	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The significant decrease in II-hydroxycorticosteroids ( II-OCS ) , adrenaline , noradrenaline , dopamine , and a tendency to the increase in histamine content were observed in the venous blood plasma .
	manualset3
165819	6	412522	7	NULL	NULL	NULL	NULL	increase	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The significant decrease in II-hydroxycorticosteroids ( II-OCS ) , adrenaline , noradrenaline , dopamine , and a tendency to the increase in histamine content were observed in the venous blood plasma .
	manualset3
165820	7	412522	7	NULL	NULL	NULL	NULL	histamine content	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The significant decrease in II-hydroxycorticosteroids ( II-OCS ) , adrenaline , noradrenaline , dopamine , and a tendency to the increase in histamine content were observed in the venous blood plasma .
	manualset3
165822	8	412522	7	NULL	NULL	NULL	NULL	venous blood plasma	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The significant decrease in II-hydroxycorticosteroids ( II-OCS ) , adrenaline , noradrenaline , dopamine , and a tendency to the increase in histamine content were observed in the venous blood plasma .
	manualset3
167231	9	412522	7	NULL	NULL	0	NULL	tendency	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The significant decrease in II-hydroxycorticosteroids ( II-OCS ) , adrenaline , noradrenaline , dopamine , and a tendency to the increase in histamine content were observed in the venous blood plasma .
	manualset3
165823	1	412523	7	NULL	NULL	NULL	NULL	gaps	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The significant gaps in knowledge , which currently preclude a more definitive evaluation of human cancer risk due to exposure to dietary acrylamide , are highlighted .
	manualset3
165824	2	412523	7	NULL	NULL	0	NULL	knowledge	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The significant gaps in knowledge , which currently preclude a more definitive evaluation of human cancer risk due to exposure to dietary acrylamide , are highlighted .
	manualset3
165825	3	412523	7	NULL	NULL	NULL	NULL	evaluation	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The significant gaps in knowledge , which currently preclude a more definitive evaluation of human cancer risk due to exposure to dietary acrylamide , are highlighted .
	manualset3
165826	4	412523	7	NULL	NULL	0	NULL	human cancer risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The significant gaps in knowledge , which currently preclude a more definitive evaluation of human cancer risk due to exposure to dietary acrylamide , are highlighted .
	manualset3
165827	5	412523	7	NULL	NULL	0	NULL	dietary acrylamide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The significant gaps in knowledge , which currently preclude a more definitive evaluation of human cancer risk due to exposure to dietary acrylamide , are highlighted .
	manualset3
166508	6	412523	7	NULL	NULL	0	NULL	exposure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The significant gaps in knowledge , which currently preclude a more definitive evaluation of human cancer risk due to exposure to dietary acrylamide , are highlighted .
	manualset3
165828	1	412524	7	NULL	NULL	NULL	NULL	elevated risk estimate	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The significantly elevated risk estimate persisted when we further excluded CRC cases within 3 years of follow-up .
	manualset3
165829	2	412524	7	NULL	NULL	0	NULL	CRC cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The significantly elevated risk estimate persisted when we further excluded CRC cases within 3 years of follow-up .
	manualset3
165830	3	412524	7	NULL	NULL	0	NULL	3 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The significantly elevated risk estimate persisted when we further excluded CRC cases within 3 years of follow-up .
	manualset3
166509	4	412524	7	NULL	NULL	0	NULL	follow-up	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The significantly elevated risk estimate persisted when we further excluded CRC cases within 3 years of follow-up .
	manualset3
165831	1	412525	7	NULL	NULL	NULL	NULL	changes	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The similar changes in heart rate and catecholamines together with the vasopressin changes suggest that , in these elderly patients with an abnormal drop of blood pressure on standing , there is no dysfunction of autonomic pathways concerned with cardiovascular function .
	manualset3
165832	2	412525	7	NULL	NULL	NULL	NULL	heart rate	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The similar changes in heart rate and catecholamines together with the vasopressin changes suggest that , in these elderly patients with an abnormal drop of blood pressure on standing , there is no dysfunction of autonomic pathways concerned with cardiovascular function .
	manualset3
165833	3	412525	7	NULL	NULL	0	NULL	catecholamines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The similar changes in heart rate and catecholamines together with the vasopressin changes suggest that , in these elderly patients with an abnormal drop of blood pressure on standing , there is no dysfunction of autonomic pathways concerned with cardiovascular function .
	manualset3
165834	4	412525	7	NULL	NULL	NULL	NULL	vasopressin changes	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The similar changes in heart rate and catecholamines together with the vasopressin changes suggest that , in these elderly patients with an abnormal drop of blood pressure on standing , there is no dysfunction of autonomic pathways concerned with cardiovascular function .
	manualset3
165835	5	412525	7	NULL	NULL	0	NULL	elderly patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The similar changes in heart rate and catecholamines together with the vasopressin changes suggest that , in these elderly patients with an abnormal drop of blood pressure on standing , there is no dysfunction of autonomic pathways concerned with cardiovascular function .
	manualset3
165836	6	412525	7	NULL	NULL	0	NULL	blood pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The similar changes in heart rate and catecholamines together with the vasopressin changes suggest that , in these elderly patients with an abnormal drop of blood pressure on standing , there is no dysfunction of autonomic pathways concerned with cardiovascular function .
	manualset3
165837	7	412525	7	NULL	NULL	NULL	NULL	dysfunction	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The similar changes in heart rate and catecholamines together with the vasopressin changes suggest that , in these elderly patients with an abnormal drop of blood pressure on standing , there is no dysfunction of autonomic pathways concerned with cardiovascular function .
	manualset3
165838	8	412525	7	NULL	NULL	0	NULL	autonomic pathways	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The similar changes in heart rate and catecholamines together with the vasopressin changes suggest that , in these elderly patients with an abnormal drop of blood pressure on standing , there is no dysfunction of autonomic pathways concerned with cardiovascular function .
	manualset3
165839	9	412525	7	NULL	NULL	0	NULL	cardiovascular function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The similar changes in heart rate and catecholamines together with the vasopressin changes suggest that , in these elderly patients with an abnormal drop of blood pressure on standing , there is no dysfunction of autonomic pathways concerned with cardiovascular function .
	manualset3
166510	10	412525	7	NULL	NULL	0	NULL	abnormal drop	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The similar changes in heart rate and catecholamines together with the vasopressin changes suggest that , in these elderly patients with an abnormal drop of blood pressure on standing , there is no dysfunction of autonomic pathways concerned with cardiovascular function .
	manualset3
166511	11	412525	7	NULL	NULL	NULL	NULL	standing	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The similar changes in heart rate and catecholamines together with the vasopressin changes suggest that , in these elderly patients with an abnormal drop of blood pressure on standing , there is no dysfunction of autonomic pathways concerned with cardiovascular function .
	manualset3
165840	1	412526	7	NULL	NULL	0	NULL	similarity	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The similarity in histologic appearance of some human cancer and normal cell strains in sponge-matrix tissue culture .
	manualset3
165841	2	412526	7	NULL	NULL	0	NULL	histologic appearance	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The similarity in histologic appearance of some human cancer and normal cell strains in sponge-matrix tissue culture .
	manualset3
165842	3	412526	7	NULL	NULL	0	NULL	human cancer cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The similarity in histologic appearance of some human cancer and normal cell strains in sponge-matrix tissue culture .
	manualset3
165843	4	412526	7	NULL	NULL	0	NULL	normal cell strains	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The similarity in histologic appearance of some human cancer and normal cell strains in sponge-matrix tissue culture .
	manualset3
165844	5	412526	7	NULL	NULL	0	NULL	sponge-matrix tissue culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The similarity in histologic appearance of some human cancer and normal cell strains in sponge-matrix tissue culture .
	manualset3
165845	1	412527	7	NULL	NULL	0	NULL	similarity	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The similarity of results for the 3 patients in this study suggest that individual differences lie in more complex stimulus processing and perhaps in qualitative aspects of perception .
	manualset3
165846	2	412527	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The similarity of results for the 3 patients in this study suggest that individual differences lie in more complex stimulus processing and perhaps in qualitative aspects of perception .
	manualset3
165847	3	412527	7	NULL	NULL	0	NULL	3 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The similarity of results for the 3 patients in this study suggest that individual differences lie in more complex stimulus processing and perhaps in qualitative aspects of perception .
	manualset3
165848	4	412527	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The similarity of results for the 3 patients in this study suggest that individual differences lie in more complex stimulus processing and perhaps in qualitative aspects of perception .
	manualset3
165849	5	412527	7	NULL	NULL	0	NULL	 complex stimulus	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The similarity of results for the 3 patients in this study suggest that individual differences lie in more complex stimulus processing and perhaps in qualitative aspects of perception .
	manualset3
165850	6	412527	7	NULL	NULL	0	NULL	qualitative aspects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The similarity of results for the 3 patients in this study suggest that individual differences lie in more complex stimulus processing and perhaps in qualitative aspects of perception .
	manualset3
165851	7	412527	7	NULL	NULL	0	NULL	perception	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The similarity of results for the 3 patients in this study suggest that individual differences lie in more complex stimulus processing and perhaps in qualitative aspects of perception .
	manualset3
165852	1	412528	7	NULL	NULL	0	NULL	 simulations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the simulations , this decline is due to a reduction in available Ca ( 2 + ) binding sites on troponin and parvalbumin .
	manualset3
165853	4	412528	7	NULL	NULL	NULL	NULL	Ca ( 2 + ) binding sites	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	According to the simulations , this decline is due to a reduction in available Ca ( 2 + ) binding sites on troponin and parvalbumin .
	manualset3
165854	5	412528	7	NULL	NULL	NULL	NULL	troponin 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	According to the simulations , this decline is due to a reduction in available Ca ( 2 + ) binding sites on troponin and parvalbumin .
	manualset3
165855	6	412528	7	NULL	NULL	NULL	NULL	parvalbumin 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	According to the simulations , this decline is due to a reduction in available Ca ( 2 + ) binding sites on troponin and parvalbumin .
	manualset3
166512	2	412528	7	NULL	NULL	NULL	NULL	decline	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	According to the simulations , this decline is due to a reduction in available Ca ( 2 + ) binding sites on troponin and parvalbumin .
	manualset3
167232	3	412528	7	NULL	NULL	NULL	NULL	 reduction	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	According to the simulations , this decline is due to a reduction in available Ca ( 2 + ) binding sites on troponin and parvalbumin .
	manualset3
165856	1	412529	7	NULL	NULL	0	NULL	 simple model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The simple model presented here , which uses plausible interatomic distances as its only free parameters , obviates the need to invoke `` iceberg '' or other water restructuring concepts which , though frequently postulated in explaining the hydrophobic interaction , are unsupported by recent experiments .
	manualset3
165857	2	412529	7	NULL	NULL	0	NULL	interatomic distances	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The simple model presented here , which uses plausible interatomic distances as its only free parameters , obviates the need to invoke `` iceberg '' or other water restructuring concepts which , though frequently postulated in explaining the hydrophobic interaction , are unsupported by recent experiments .
	manualset3
165858	3	412529	7	NULL	NULL	0	NULL	free parameters	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The simple model presented here , which uses plausible interatomic distances as its only free parameters , obviates the need to invoke `` iceberg '' or other water restructuring concepts which , though frequently postulated in explaining the hydrophobic interaction , are unsupported by recent experiments .
	manualset3
165859	4	412529	7	NULL	NULL	0	NULL	 iceberg	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The simple model presented here , which uses plausible interatomic distances as its only free parameters , obviates the need to invoke `` iceberg '' or other water restructuring concepts which , though frequently postulated in explaining the hydrophobic interaction , are unsupported by recent experiments .
	manualset3
165860	5	412529	7	NULL	NULL	0	NULL	water restructuring concepts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The simple model presented here , which uses plausible interatomic distances as its only free parameters , obviates the need to invoke `` iceberg '' or other water restructuring concepts which , though frequently postulated in explaining the hydrophobic interaction , are unsupported by recent experiments .
	manualset3
165861	6	412529	7	NULL	NULL	0	NULL	hydrophobic interaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The simple model presented here , which uses plausible interatomic distances as its only free parameters , obviates the need to invoke `` iceberg '' or other water restructuring concepts which , though frequently postulated in explaining the hydrophobic interaction , are unsupported by recent experiments .
	manualset3
165862	7	412529	7	NULL	NULL	0	NULL	 experiments 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The simple model presented here , which uses plausible interatomic distances as its only free parameters , obviates the need to invoke `` iceberg '' or other water restructuring concepts which , though frequently postulated in explaining the hydrophobic interaction , are unsupported by recent experiments .
	manualset3
165863	1	412530	7	NULL	NULL	0	NULL	bacterial enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The simplest bacterial enzyme contains an endonuclease domain ( endoND ) and a dsRNA binding domain ( dsRBD ) .
	manualset3
165864	2	412530	7	NULL	NULL	0	NULL	endonuclease domain ( endoND )	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The simplest bacterial enzyme contains an endonuclease domain ( endoND ) and a dsRNA binding domain ( dsRBD ) .
	manualset3
165865	3	412530	7	NULL	NULL	0	NULL	dsRNA binding domain ( dsRBD )	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The simplest bacterial enzyme contains an endonuclease domain ( endoND ) and a dsRNA binding domain ( dsRBD ) .
	manualset3
165873	1	412531	7	NULL	NULL	0	NULL	simplicity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The simplicity of this method , saving the chemicals without a quality loss , a possibility of tissue processing through paraffin and celloidin as well as having histological slides 5-6 hours after cutting material allow one to recommend the above apparatus for the practical use .
	manualset3
165874	2	412531	7	NULL	NULL	NULL	NULL	method	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The simplicity of this method , saving the chemicals without a quality loss , a possibility of tissue processing through paraffin and celloidin as well as having histological slides 5-6 hours after cutting material allow one to recommend the above apparatus for the practical use .
	manualset3
165875	3	412531	7	NULL	NULL	0	NULL	chemicals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The simplicity of this method , saving the chemicals without a quality loss , a possibility of tissue processing through paraffin and celloidin as well as having histological slides 5-6 hours after cutting material allow one to recommend the above apparatus for the practical use .
	manualset3
165876	4	412531	7	NULL	NULL	NULL	NULL	tissue processing	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The simplicity of this method , saving the chemicals without a quality loss , a possibility of tissue processing through paraffin and celloidin as well as having histological slides 5-6 hours after cutting material allow one to recommend the above apparatus for the practical use .
	manualset3
165877	5	412531	7	NULL	NULL	0	NULL	paraffin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The simplicity of this method , saving the chemicals without a quality loss , a possibility of tissue processing through paraffin and celloidin as well as having histological slides 5-6 hours after cutting material allow one to recommend the above apparatus for the practical use .
	manualset3
165878	6	412531	7	NULL	NULL	0	NULL	celloidin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The simplicity of this method , saving the chemicals without a quality loss , a possibility of tissue processing through paraffin and celloidin as well as having histological slides 5-6 hours after cutting material allow one to recommend the above apparatus for the practical use .
	manualset3
165879	7	412531	7	NULL	NULL	0	NULL	histological slides	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The simplicity of this method , saving the chemicals without a quality loss , a possibility of tissue processing through paraffin and celloidin as well as having histological slides 5-6 hours after cutting material allow one to recommend the above apparatus for the practical use .
	manualset3
165880	8	412531	7	NULL	NULL	0	NULL	5-6 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The simplicity of this method , saving the chemicals without a quality loss , a possibility of tissue processing through paraffin and celloidin as well as having histological slides 5-6 hours after cutting material allow one to recommend the above apparatus for the practical use .
	manualset3
165881	9	412531	7	NULL	NULL	0	NULL	cutting material 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The simplicity of this method , saving the chemicals without a quality loss , a possibility of tissue processing through paraffin and celloidin as well as having histological slides 5-6 hours after cutting material allow one to recommend the above apparatus for the practical use .
	manualset3
165882	10	412531	7	NULL	NULL	NULL	NULL	apparatus	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The simplicity of this method , saving the chemicals without a quality loss , a possibility of tissue processing through paraffin and celloidin as well as having histological slides 5-6 hours after cutting material allow one to recommend the above apparatus for the practical use .
	manualset3
165883	11	412531	7	NULL	NULL	0	NULL	practical use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The simplicity of this method , saving the chemicals without a quality loss , a possibility of tissue processing through paraffin and celloidin as well as having histological slides 5-6 hours after cutting material allow one to recommend the above apparatus for the practical use .
	manualset3
166498	12	412531	7	NULL	NULL	0	NULL	 quality loss 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The simplicity of this method , saving the chemicals without a quality loss , a possibility of tissue processing through paraffin and celloidin as well as having histological slides 5-6 hours after cutting material allow one to recommend the above apparatus for the practical use .
	manualset3
166499	13	412531	7	NULL	NULL	0	NULL	possibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The simplicity of this method , saving the chemicals without a quality loss , a possibility of tissue processing through paraffin and celloidin as well as having histological slides 5-6 hours after cutting material allow one to recommend the above apparatus for the practical use .
	manualset3
166500	14	412531	7	NULL	NULL	0	NULL	one	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The simplicity of this method , saving the chemicals without a quality loss , a possibility of tissue processing through paraffin and celloidin as well as having histological slides 5-6 hours after cutting material allow one to recommend the above apparatus for the practical use .
	manualset3
165884	1	412532	7	NULL	NULL	0	NULL	lack	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The simultaneous lack of oxygen and glucose resulted in a very pronounced release of the 3H-amine .
	manualset3
165885	2	412532	7	NULL	NULL	0	NULL	oxygen	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The simultaneous lack of oxygen and glucose resulted in a very pronounced release of the 3H-amine .
	manualset3
165886	3	412532	7	NULL	NULL	0	NULL	glucose	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The simultaneous lack of oxygen and glucose resulted in a very pronounced release of the 3H-amine .
	manualset3
165887	4	412532	7	NULL	NULL	0	NULL	 release	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The simultaneous lack of oxygen and glucose resulted in a very pronounced release of the 3H-amine .
	manualset3
165888	5	412532	7	NULL	NULL	0	NULL	3H-amine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The simultaneous lack of oxygen and glucose resulted in a very pronounced release of the 3H-amine .
	manualset3
165889	1	412533	7	NULL	NULL	NULL	NULL	supply	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The simultaneous supply of dietary polyunsaturated fatty acids and nucleotides was beneficial in the reversal of abnormalities of the lipid metabolism , in this experimental model of liver cirrhosis .
	manualset3
165890	2	412533	7	NULL	NULL	0	NULL	dietary polyunsaturated fatty acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The simultaneous supply of dietary polyunsaturated fatty acids and nucleotides was beneficial in the reversal of abnormalities of the lipid metabolism , in this experimental model of liver cirrhosis .
	manualset3
165891	3	412533	7	NULL	NULL	0	NULL	nucleotides	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The simultaneous supply of dietary polyunsaturated fatty acids and nucleotides was beneficial in the reversal of abnormalities of the lipid metabolism , in this experimental model of liver cirrhosis .
	manualset3
165892	4	412533	7	NULL	NULL	NULL	NULL	reversal	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The simultaneous supply of dietary polyunsaturated fatty acids and nucleotides was beneficial in the reversal of abnormalities of the lipid metabolism , in this experimental model of liver cirrhosis .
	manualset3
165893	5	412533	7	NULL	NULL	0	NULL	abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The simultaneous supply of dietary polyunsaturated fatty acids and nucleotides was beneficial in the reversal of abnormalities of the lipid metabolism , in this experimental model of liver cirrhosis .
	manualset3
165894	6	412533	7	NULL	NULL	0	NULL	lipid metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The simultaneous supply of dietary polyunsaturated fatty acids and nucleotides was beneficial in the reversal of abnormalities of the lipid metabolism , in this experimental model of liver cirrhosis .
	manualset3
165895	7	412533	7	NULL	NULL	0	NULL	experimental model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The simultaneous supply of dietary polyunsaturated fatty acids and nucleotides was beneficial in the reversal of abnormalities of the lipid metabolism , in this experimental model of liver cirrhosis .
	manualset3
165896	8	412533	7	NULL	NULL	0	NULL	liver cirrhosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The simultaneous supply of dietary polyunsaturated fatty acids and nucleotides was beneficial in the reversal of abnormalities of the lipid metabolism , in this experimental model of liver cirrhosis .
	manualset3
165897	1	412534	7	NULL	NULL	0	NULL	size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The size changes were fully reversible and could be elicited repeatedly by feeding .
	manualset3
165899	3	412534	7	NULL	NULL	0	NULL	feeding 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The size changes were fully reversible and could be elicited repeatedly by feeding .
	manualset3
165900	1	412535	7	NULL	NULL	0	NULL	traditional immunization procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the traditional immunization procedure , after the first injection of the sample A ( emulsion of aimed antigen and Freund 's complete adjuvant ) to immunize rabbit , successive injections of the sample B ( emulsion of aimed antigen and Freund 's incomplete adjuvant ) were followed every 2-4 weeks .
	manualset3
165901	2	412535	7	NULL	NULL	0	NULL	first injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the traditional immunization procedure , after the first injection of the sample A ( emulsion of aimed antigen and Freund 's complete adjuvant ) to immunize rabbit , successive injections of the sample B ( emulsion of aimed antigen and Freund 's incomplete adjuvant ) were followed every 2-4 weeks .
	manualset3
165902	3	412535	7	NULL	NULL	0	NULL	sample A	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the traditional immunization procedure , after the first injection of the sample A ( emulsion of aimed antigen and Freund 's complete adjuvant ) to immunize rabbit , successive injections of the sample B ( emulsion of aimed antigen and Freund 's incomplete adjuvant ) were followed every 2-4 weeks .
	manualset3
165903	4	412535	7	NULL	NULL	0	NULL	emulsion	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the traditional immunization procedure , after the first injection of the sample A ( emulsion of aimed antigen and Freund 's complete adjuvant ) to immunize rabbit , successive injections of the sample B ( emulsion of aimed antigen and Freund 's incomplete adjuvant ) were followed every 2-4 weeks .
	manualset3
165904	5	412535	7	NULL	NULL	NULL	NULL	aimed antigen 	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	According to the traditional immunization procedure , after the first injection of the sample A ( emulsion of aimed antigen and Freund 's complete adjuvant ) to immunize rabbit , successive injections of the sample B ( emulsion of aimed antigen and Freund 's incomplete adjuvant ) were followed every 2-4 weeks .
	manualset3
165905	6	412535	7	NULL	NULL	0	NULL	 Freund 's complete adjuvant	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the traditional immunization procedure , after the first injection of the sample A ( emulsion of aimed antigen and Freund 's complete adjuvant ) to immunize rabbit , successive injections of the sample B ( emulsion of aimed antigen and Freund 's incomplete adjuvant ) were followed every 2-4 weeks .
	manualset3
165906	7	412535	7	NULL	NULL	0	NULL	 rabbit	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the traditional immunization procedure , after the first injection of the sample A ( emulsion of aimed antigen and Freund 's complete adjuvant ) to immunize rabbit , successive injections of the sample B ( emulsion of aimed antigen and Freund 's incomplete adjuvant ) were followed every 2-4 weeks .
	manualset3
165907	8	412535	7	NULL	NULL	0	NULL	injections 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the traditional immunization procedure , after the first injection of the sample A ( emulsion of aimed antigen and Freund 's complete adjuvant ) to immunize rabbit , successive injections of the sample B ( emulsion of aimed antigen and Freund 's incomplete adjuvant ) were followed every 2-4 weeks .
	manualset3
165908	9	412535	7	NULL	NULL	0	NULL	sample B	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the traditional immunization procedure , after the first injection of the sample A ( emulsion of aimed antigen and Freund 's complete adjuvant ) to immunize rabbit , successive injections of the sample B ( emulsion of aimed antigen and Freund 's incomplete adjuvant ) were followed every 2-4 weeks .
	manualset3
165909	10	412535	7	NULL	NULL	0	NULL	emulsion	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the traditional immunization procedure , after the first injection of the sample A ( emulsion of aimed antigen and Freund 's complete adjuvant ) to immunize rabbit , successive injections of the sample B ( emulsion of aimed antigen and Freund 's incomplete adjuvant ) were followed every 2-4 weeks .
	manualset3
165910	11	412535	7	NULL	NULL	0	NULL	aimed antigen	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the traditional immunization procedure , after the first injection of the sample A ( emulsion of aimed antigen and Freund 's complete adjuvant ) to immunize rabbit , successive injections of the sample B ( emulsion of aimed antigen and Freund 's incomplete adjuvant ) were followed every 2-4 weeks .
	manualset3
165911	12	412535	7	NULL	NULL	0	NULL	Freund 's incomplete adjuvant	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the traditional immunization procedure , after the first injection of the sample A ( emulsion of aimed antigen and Freund 's complete adjuvant ) to immunize rabbit , successive injections of the sample B ( emulsion of aimed antigen and Freund 's incomplete adjuvant ) were followed every 2-4 weeks .
	manualset3
165912	13	412535	7	NULL	NULL	0	NULL	2-4 weeks 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the traditional immunization procedure , after the first injection of the sample A ( emulsion of aimed antigen and Freund 's complete adjuvant ) to immunize rabbit , successive injections of the sample B ( emulsion of aimed antigen and Freund 's incomplete adjuvant ) were followed every 2-4 weeks .
	manualset3
165913	1	412536	7	NULL	NULL	0	NULL	size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The size of the band gap can be tuned by the position of the antidots and the distance D between the two nearest antidots .
	manualset3
165914	2	412536	7	NULL	NULL	0	NULL	 band gap 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The size of the band gap can be tuned by the position of the antidots and the distance D between the two nearest antidots .
	manualset3
165915	3	412536	7	NULL	NULL	0	NULL	 position 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The size of the band gap can be tuned by the position of the antidots and the distance D between the two nearest antidots .
	manualset3
165916	4	412536	7	NULL	NULL	0	NULL	antidots	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The size of the band gap can be tuned by the position of the antidots and the distance D between the two nearest antidots .
	manualset3
165917	5	412536	7	NULL	NULL	0	NULL	distance D	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The size of the band gap can be tuned by the position of the antidots and the distance D between the two nearest antidots .
	manualset3
165918	6	412536	7	NULL	NULL	NULL	NULL	antidots	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The size of the band gap can be tuned by the position of the antidots and the distance D between the two nearest antidots .
	manualset3
165919	1	412537	7	NULL	NULL	0	NULL	 size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The size of the soma area was not correlated to the dendritic field size and increased from 100 to 150 microm ( 2 ) near the fovea to 150-300 microm ( 2 ) at the retinal margin .
	manualset3
165920	2	412537	7	NULL	NULL	0	NULL	soma area	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The size of the soma area was not correlated to the dendritic field size and increased from 100 to 150 microm ( 2 ) near the fovea to 150-300 microm ( 2 ) at the retinal margin .
	manualset3
165921	3	412537	7	NULL	NULL	0	NULL	dendritic field size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The size of the soma area was not correlated to the dendritic field size and increased from 100 to 150 microm ( 2 ) near the fovea to 150-300 microm ( 2 ) at the retinal margin .
	manualset3
165922	4	412537	7	NULL	NULL	0	NULL	100 to 150 microm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The size of the soma area was not correlated to the dendritic field size and increased from 100 to 150 microm ( 2 ) near the fovea to 150-300 microm ( 2 ) at the retinal margin .
	manualset3
165923	5	412537	7	NULL	NULL	0	NULL	fovea	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The size of the soma area was not correlated to the dendritic field size and increased from 100 to 150 microm ( 2 ) near the fovea to 150-300 microm ( 2 ) at the retinal margin .
	manualset3
165924	6	412537	7	NULL	NULL	0	NULL	150-300 microm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The size of the soma area was not correlated to the dendritic field size and increased from 100 to 150 microm ( 2 ) near the fovea to 150-300 microm ( 2 ) at the retinal margin .
	manualset3
165925	7	412537	7	NULL	NULL	0	NULL	retinal margin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The size of the soma area was not correlated to the dendritic field size and increased from 100 to 150 microm ( 2 ) near the fovea to 150-300 microm ( 2 ) at the retinal margin .
	manualset3
165926	1	412538	7	NULL	NULL	0	NULL	skeletal muscle ryanodine receptor ( RYR1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The skeletal muscle ryanodine receptor ( RYR1 ) belongs to a family of calcium release channels that are expressed in different tissues .
	manualset3
165927	2	412538	7	NULL	NULL	0	NULL	family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The skeletal muscle ryanodine receptor ( RYR1 ) belongs to a family of calcium release channels that are expressed in different tissues .
	manualset3
165928	3	412538	7	NULL	NULL	0	NULL	calcium release channels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The skeletal muscle ryanodine receptor ( RYR1 ) belongs to a family of calcium release channels that are expressed in different tissues .
	manualset3
165929	4	412538	7	NULL	NULL	NULL	NULL	different tissues	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The skeletal muscle ryanodine receptor ( RYR1 ) belongs to a family of calcium release channels that are expressed in different tissues .
	manualset3
165930	1	412539	7	NULL	NULL	0	NULL	skin biopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The skin biopsy showed a flattened epidermis and a proliferation of collagen bundles in the dermis .
	manualset3
165931	2	412539	7	NULL	NULL	0	NULL	flattened epidermis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The skin biopsy showed a flattened epidermis and a proliferation of collagen bundles in the dermis .
	manualset3
165932	3	412539	7	NULL	NULL	0	NULL	proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The skin biopsy showed a flattened epidermis and a proliferation of collagen bundles in the dermis .
	manualset3
165933	4	412539	7	NULL	NULL	0	NULL	collagen bundles	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The skin biopsy showed a flattened epidermis and a proliferation of collagen bundles in the dermis .
	manualset3
165934	5	412539	7	NULL	NULL	NULL	NULL	dermis	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The skin biopsy showed a flattened epidermis and a proliferation of collagen bundles in the dermis .
	manualset3
165935	1	412540	7	NULL	NULL	0	NULL	sled dog genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The sled dog genome is enhanced by differential contributions from four non-admixed breeds ( Alaskan Malamute , Siberian Husky , German Shorthaired Pointer , and Borzoi ) .
	manualset3
165936	2	412540	7	NULL	NULL	0	NULL	differential contributions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The sled dog genome is enhanced by differential contributions from four non-admixed breeds ( Alaskan Malamute , Siberian Husky , German Shorthaired Pointer , and Borzoi ) .
	manualset3
165937	3	412540	7	NULL	NULL	0	NULL	four	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The sled dog genome is enhanced by differential contributions from four non-admixed breeds ( Alaskan Malamute , Siberian Husky , German Shorthaired Pointer , and Borzoi ) .
	manualset3
165938	4	412540	7	NULL	NULL	0	NULL	non-admixed breeds	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The sled dog genome is enhanced by differential contributions from four non-admixed breeds ( Alaskan Malamute , Siberian Husky , German Shorthaired Pointer , and Borzoi ) .
	manualset3
165939	5	412540	7	NULL	NULL	0	NULL	Alaskan Malamute 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The sled dog genome is enhanced by differential contributions from four non-admixed breeds ( Alaskan Malamute , Siberian Husky , German Shorthaired Pointer , and Borzoi ) .
	manualset3
165940	6	412540	7	NULL	NULL	0	NULL	Siberian Husky	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The sled dog genome is enhanced by differential contributions from four non-admixed breeds ( Alaskan Malamute , Siberian Husky , German Shorthaired Pointer , and Borzoi ) .
	manualset3
165941	7	412540	7	NULL	NULL	0	NULL	German Shorthaired Pointer	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The sled dog genome is enhanced by differential contributions from four non-admixed breeds ( Alaskan Malamute , Siberian Husky , German Shorthaired Pointer , and Borzoi ) .
	manualset3
165942	8	412540	7	NULL	NULL	0	NULL	Borzoi	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The sled dog genome is enhanced by differential contributions from four non-admixed breeds ( Alaskan Malamute , Siberian Husky , German Shorthaired Pointer , and Borzoi ) .
	manualset3
165943	1	412541	7	NULL	NULL	0	NULL	 slide and step osteotomies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The slide and step osteotomies were tested on six bilateral pairs of cadaveric femora with cyclic shear load of constant amplitude for 100 cycles in both a superior direction to represent standing and 60 degrees of hip flexion to represent a squat stance .
	manualset3
165944	2	412541	7	NULL	NULL	0	NULL	six bilateral pairs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The slide and step osteotomies were tested on six bilateral pairs of cadaveric femora with cyclic shear load of constant amplitude for 100 cycles in both a superior direction to represent standing and 60 degrees of hip flexion to represent a squat stance .
	manualset3
165945	3	412541	7	NULL	NULL	0	NULL	cadaveric femora 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The slide and step osteotomies were tested on six bilateral pairs of cadaveric femora with cyclic shear load of constant amplitude for 100 cycles in both a superior direction to represent standing and 60 degrees of hip flexion to represent a squat stance .
	manualset3
165946	4	412541	7	NULL	NULL	0	NULL	cyclic shear load	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The slide and step osteotomies were tested on six bilateral pairs of cadaveric femora with cyclic shear load of constant amplitude for 100 cycles in both a superior direction to represent standing and 60 degrees of hip flexion to represent a squat stance .
	manualset3
165947	5	412541	7	NULL	NULL	0	NULL	constant amplitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The slide and step osteotomies were tested on six bilateral pairs of cadaveric femora with cyclic shear load of constant amplitude for 100 cycles in both a superior direction to represent standing and 60 degrees of hip flexion to represent a squat stance .
	manualset3
165948	6	412541	7	NULL	NULL	0	NULL	100 cycles	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The slide and step osteotomies were tested on six bilateral pairs of cadaveric femora with cyclic shear load of constant amplitude for 100 cycles in both a superior direction to represent standing and 60 degrees of hip flexion to represent a squat stance .
	manualset3
165949	7	412541	7	NULL	NULL	0	NULL	superior direction	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The slide and step osteotomies were tested on six bilateral pairs of cadaveric femora with cyclic shear load of constant amplitude for 100 cycles in both a superior direction to represent standing and 60 degrees of hip flexion to represent a squat stance .
	manualset3
165950	8	412541	7	NULL	NULL	0	NULL	standing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The slide and step osteotomies were tested on six bilateral pairs of cadaveric femora with cyclic shear load of constant amplitude for 100 cycles in both a superior direction to represent standing and 60 degrees of hip flexion to represent a squat stance .
	manualset3
165951	9	412541	7	NULL	NULL	0	NULL	 60 degrees	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The slide and step osteotomies were tested on six bilateral pairs of cadaveric femora with cyclic shear load of constant amplitude for 100 cycles in both a superior direction to represent standing and 60 degrees of hip flexion to represent a squat stance .
	manualset3
165952	10	412541	7	NULL	NULL	0	NULL	hip flexion	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The slide and step osteotomies were tested on six bilateral pairs of cadaveric femora with cyclic shear load of constant amplitude for 100 cycles in both a superior direction to represent standing and 60 degrees of hip flexion to represent a squat stance .
	manualset3
165953	11	412541	7	NULL	NULL	0	NULL	squat stance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The slide and step osteotomies were tested on six bilateral pairs of cadaveric femora with cyclic shear load of constant amplitude for 100 cycles in both a superior direction to represent standing and 60 degrees of hip flexion to represent a squat stance .
	manualset3
165954	1	412542	7	NULL	NULL	0	NULL	slight pain group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The slight pain group had no abnormalities except for mild cardiovagal dysfunction .
	manualset3
165955	2	412542	7	NULL	NULL	0	NULL	abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The slight pain group had no abnormalities except for mild cardiovagal dysfunction .
	manualset3
165956	3	412542	7	NULL	NULL	0	NULL	 mild cardiovagal dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The slight pain group had no abnormalities except for mild cardiovagal dysfunction .
	manualset3
165957	1	412543	7	NULL	NULL	0	NULL	slope ( coefficient ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The slope ( coefficient ) of the different regression line , however , clearly decreased with the reduction in skin temperature except for 27-25 degrees C ( p ) 0.05 ) .
	manualset3
165958	2	412543	7	NULL	NULL	0	NULL	regression line	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The slope ( coefficient ) of the different regression line , however , clearly decreased with the reduction in skin temperature except for 27-25 degrees C ( p ) 0.05 ) .
	manualset3
165959	3	412543	7	NULL	NULL	0	NULL	 reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The slope ( coefficient ) of the different regression line , however , clearly decreased with the reduction in skin temperature except for 27-25 degrees C ( p ) 0.05 ) .
	manualset3
165960	4	412543	7	NULL	NULL	0	NULL	skin temperature	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The slope ( coefficient ) of the different regression line , however , clearly decreased with the reduction in skin temperature except for 27-25 degrees C ( p ) 0.05 ) .
	manualset3
165961	5	412543	7	NULL	NULL	0	NULL	27-25 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The slope ( coefficient ) of the different regression line , however , clearly decreased with the reduction in skin temperature except for 27-25 degrees C ( p ) 0.05 ) .
	manualset3
165962	6	412543	7	NULL	NULL	0	NULL	( p ) 0.05 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The slope ( coefficient ) of the different regression line , however , clearly decreased with the reduction in skin temperature except for 27-25 degrees C ( p ) 0.05 ) .
	manualset3
165963	1	412544	7	NULL	NULL	0	NULL	slope	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The slope and y intercept of this relationship was derived by linear regression and then used to predict an idealized MCHC , which in combination with the MCH was used to derive a predicted MCV .
	manualset3
165964	2	412544	7	NULL	NULL	0	NULL	 y intercept 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The slope and y intercept of this relationship was derived by linear regression and then used to predict an idealized MCHC , which in combination with the MCH was used to derive a predicted MCV .
	manualset3
165965	3	412544	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The slope and y intercept of this relationship was derived by linear regression and then used to predict an idealized MCHC , which in combination with the MCH was used to derive a predicted MCV .
	manualset3
165966	4	412544	7	NULL	NULL	0	NULL	 linear regression	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The slope and y intercept of this relationship was derived by linear regression and then used to predict an idealized MCHC , which in combination with the MCH was used to derive a predicted MCV .
	manualset3
165967	5	412544	7	NULL	NULL	0	NULL	idealized MCHC	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The slope and y intercept of this relationship was derived by linear regression and then used to predict an idealized MCHC , which in combination with the MCH was used to derive a predicted MCV .
	manualset3
165968	6	412544	7	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The slope and y intercept of this relationship was derived by linear regression and then used to predict an idealized MCHC , which in combination with the MCH was used to derive a predicted MCV .
	manualset3
165969	7	412544	7	NULL	NULL	0	NULL	MCH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The slope and y intercept of this relationship was derived by linear regression and then used to predict an idealized MCHC , which in combination with the MCH was used to derive a predicted MCV .
	manualset3
165970	8	412544	7	NULL	NULL	0	NULL	predicted MCV	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The slope and y intercept of this relationship was derived by linear regression and then used to predict an idealized MCHC , which in combination with the MCH was used to derive a predicted MCV .
	manualset3
165971	1	412545	7	NULL	NULL	NULL	NULL	slow axonal transport	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The slow axonal transport of cytoskeletal proteins .
	manualset3
165972	2	412545	7	NULL	NULL	0	NULL	cytoskeletal proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The slow axonal transport of cytoskeletal proteins .
	manualset3
165973	1	412546	7	NULL	NULL	0	NULL	slow rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The slow rate of mtDNA evolution in turtles poses a limitation on the levels of intraspecific variation detectable by conventional restriction fragment surveys .
	manualset3
165974	2	412546	7	NULL	NULL	0	NULL	mtDNA evolution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The slow rate of mtDNA evolution in turtles poses a limitation on the levels of intraspecific variation detectable by conventional restriction fragment surveys .
	manualset3
165975	3	412546	7	NULL	NULL	0	NULL	 turtles	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The slow rate of mtDNA evolution in turtles poses a limitation on the levels of intraspecific variation detectable by conventional restriction fragment surveys .
	manualset3
165976	4	412546	7	NULL	NULL	0	NULL	limitation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The slow rate of mtDNA evolution in turtles poses a limitation on the levels of intraspecific variation detectable by conventional restriction fragment surveys .
	manualset3
165977	5	412546	7	NULL	NULL	0	NULL	 levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The slow rate of mtDNA evolution in turtles poses a limitation on the levels of intraspecific variation detectable by conventional restriction fragment surveys .
	manualset3
165978	6	412546	7	NULL	NULL	0	NULL	intraspecific variation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The slow rate of mtDNA evolution in turtles poses a limitation on the levels of intraspecific variation detectable by conventional restriction fragment surveys .
	manualset3
165979	7	412546	7	NULL	NULL	0	NULL	conventional restriction fragment surveys	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The slow rate of mtDNA evolution in turtles poses a limitation on the levels of intraspecific variation detectable by conventional restriction fragment surveys .
	manualset3
165980	1	412547	7	NULL	NULL	0	NULL	slower mitosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The slower mitosis in mutant cells did not result in premature cytokinesis and cell death , further suggesting that cell-cycle control mechanisms `` sense '' the mitotic slowdown , possibly by monitoring MT dynamics directly .
	manualset3
165981	2	412547	7	NULL	NULL	0	NULL	mutant cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The slower mitosis in mutant cells did not result in premature cytokinesis and cell death , further suggesting that cell-cycle control mechanisms `` sense '' the mitotic slowdown , possibly by monitoring MT dynamics directly .
	manualset3
165982	3	412547	7	NULL	NULL	0	NULL	premature cytokinesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The slower mitosis in mutant cells did not result in premature cytokinesis and cell death , further suggesting that cell-cycle control mechanisms `` sense '' the mitotic slowdown , possibly by monitoring MT dynamics directly .
	manualset3
165983	4	412547	7	NULL	NULL	0	NULL	cell death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The slower mitosis in mutant cells did not result in premature cytokinesis and cell death , further suggesting that cell-cycle control mechanisms `` sense '' the mitotic slowdown , possibly by monitoring MT dynamics directly .
	manualset3
165984	5	412547	7	NULL	NULL	0	NULL	cell-cycle control mechanisms 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The slower mitosis in mutant cells did not result in premature cytokinesis and cell death , further suggesting that cell-cycle control mechanisms `` sense '' the mitotic slowdown , possibly by monitoring MT dynamics directly .
	manualset3
165986	7	412547	7	NULL	NULL	0	NULL	mitotic slowdown	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The slower mitosis in mutant cells did not result in premature cytokinesis and cell death , further suggesting that cell-cycle control mechanisms `` sense '' the mitotic slowdown , possibly by monitoring MT dynamics directly .
	manualset3
165987	8	412547	7	NULL	NULL	NULL	NULL	MT dynamics	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The slower mitosis in mutant cells did not result in premature cytokinesis and cell death , further suggesting that cell-cycle control mechanisms `` sense '' the mitotic slowdown , possibly by monitoring MT dynamics directly .
	manualset3
165988	1	412548	7	NULL	NULL	0	NULL	slower protein relaxation rate tau	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The slower protein relaxation rate tau ( 22 ) in DHP-NO relative to HHMbNO implies less effective trapping in the docking site of the distal pocket and is consistent with a greater yield for the fast geminate process .
	manualset3
165989	2	412548	7	NULL	NULL	0	NULL	DHP-NO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The slower protein relaxation rate tau ( 22 ) in DHP-NO relative to HHMbNO implies less effective trapping in the docking site of the distal pocket and is consistent with a greater yield for the fast geminate process .
	manualset3
165990	3	412548	7	NULL	NULL	0	NULL	HHMbNO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The slower protein relaxation rate tau ( 22 ) in DHP-NO relative to HHMbNO implies less effective trapping in the docking site of the distal pocket and is consistent with a greater yield for the fast geminate process .
	manualset3
165991	4	412548	7	NULL	NULL	0	NULL	trapping	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The slower protein relaxation rate tau ( 22 ) in DHP-NO relative to HHMbNO implies less effective trapping in the docking site of the distal pocket and is consistent with a greater yield for the fast geminate process .
	manualset3
165992	5	412548	7	NULL	NULL	0	NULL	docking site	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The slower protein relaxation rate tau ( 22 ) in DHP-NO relative to HHMbNO implies less effective trapping in the docking site of the distal pocket and is consistent with a greater yield for the fast geminate process .
	manualset3
165993	6	412548	7	NULL	NULL	0	NULL	distal pocket	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The slower protein relaxation rate tau ( 22 ) in DHP-NO relative to HHMbNO implies less effective trapping in the docking site of the distal pocket and is consistent with a greater yield for the fast geminate process .
	manualset3
165994	7	412548	7	NULL	NULL	0	NULL	greater yield 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The slower protein relaxation rate tau ( 22 ) in DHP-NO relative to HHMbNO implies less effective trapping in the docking site of the distal pocket and is consistent with a greater yield for the fast geminate process .
	manualset3
165995	8	412548	7	NULL	NULL	0	NULL	fast geminate process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The slower protein relaxation rate tau ( 22 ) in DHP-NO relative to HHMbNO implies less effective trapping in the docking site of the distal pocket and is consistent with a greater yield for the fast geminate process .
	manualset3
165996	1	412549	7	NULL	NULL	0	NULL	small peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The small peptides formed in the presence of reserpine in vitro are also produced in vivo .
	manualset3
165997	2	412549	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The small peptides formed in the presence of reserpine in vitro are also produced in vivo .
	manualset3
165998	3	412549	7	NULL	NULL	0	NULL	 reserpine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The small peptides formed in the presence of reserpine in vitro are also produced in vivo .
	manualset3
165999	1	412550	7	NULL	NULL	NULL	NULL	 Snail1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Accordingly , Snail1 and Twist cooperate in the induction of Zeb1 : co-transfection of both cDNAs is required for the maximal expression of ZEB1 mRNA .
	manualset3
166000	2	412550	7	NULL	NULL	0	NULL	 induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , Snail1 and Twist cooperate in the induction of Zeb1 : co-transfection of both cDNAs is required for the maximal expression of ZEB1 mRNA .
	manualset3
166001	3	412550	7	NULL	NULL	0	NULL	Zeb1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , Snail1 and Twist cooperate in the induction of Zeb1 : co-transfection of both cDNAs is required for the maximal expression of ZEB1 mRNA .
	manualset3
166002	4	412550	7	NULL	NULL	0	NULL	 co-transfection 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , Snail1 and Twist cooperate in the induction of Zeb1 : co-transfection of both cDNAs is required for the maximal expression of ZEB1 mRNA .
	manualset3
166003	5	412550	7	NULL	NULL	NULL	NULL	cDNAs	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Accordingly , Snail1 and Twist cooperate in the induction of Zeb1 : co-transfection of both cDNAs is required for the maximal expression of ZEB1 mRNA .
	manualset3
166004	6	412550	7	NULL	NULL	0	NULL	maximal expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , Snail1 and Twist cooperate in the induction of Zeb1 : co-transfection of both cDNAs is required for the maximal expression of ZEB1 mRNA .
	manualset3
166005	7	412550	7	NULL	NULL	NULL	NULL	ZEB1 mRNA	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Accordingly , Snail1 and Twist cooperate in the induction of Zeb1 : co-transfection of both cDNAs is required for the maximal expression of ZEB1 mRNA .
	manualset3
166501	8	412550	7	NULL	NULL	0	NULL	Twist 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , Snail1 and Twist cooperate in the induction of Zeb1 : co-transfection of both cDNAs is required for the maximal expression of ZEB1 mRNA .
	manualset3
166006	1	412551	7	NULL	NULL	0	NULL	socially aggressive congener	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The socially aggressive congener Geospiza magnirostris ( large ground finch ) , singing in the same frequency band ( 2-4 kHz ) , colonized Daphne in 1983 and increased in numbers .
	manualset3
166007	2	412551	7	NULL	NULL	0	NULL	Geospiza magnirostris ( large ground finch )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The socially aggressive congener Geospiza magnirostris ( large ground finch ) , singing in the same frequency band ( 2-4 kHz ) , colonized Daphne in 1983 and increased in numbers .
	manualset3
166008	3	412551	7	NULL	NULL	0	NULL	frequency band	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The socially aggressive congener Geospiza magnirostris ( large ground finch ) , singing in the same frequency band ( 2-4 kHz ) , colonized Daphne in 1983 and increased in numbers .
	manualset3
166009	4	412551	7	NULL	NULL	0	NULL	2-4 kHz	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The socially aggressive congener Geospiza magnirostris ( large ground finch ) , singing in the same frequency band ( 2-4 kHz ) , colonized Daphne in 1983 and increased in numbers .
	manualset3
166010	5	412551	7	NULL	NULL	0	NULL	Daphne	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The socially aggressive congener Geospiza magnirostris ( large ground finch ) , singing in the same frequency band ( 2-4 kHz ) , colonized Daphne in 1983 and increased in numbers .
	manualset3
166011	6	412551	7	NULL	NULL	NULL	NULL	1983	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The socially aggressive congener Geospiza magnirostris ( large ground finch ) , singing in the same frequency band ( 2-4 kHz ) , colonized Daphne in 1983 and increased in numbers .
	manualset3
166012	7	412551	7	NULL	NULL	0	NULL	numbers 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The socially aggressive congener Geospiza magnirostris ( large ground finch ) , singing in the same frequency band ( 2-4 kHz ) , colonized Daphne in 1983 and increased in numbers .
	manualset3
166013	1	412552	7	NULL	NULL	0	NULL	soft contact lenses	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The soft contact lenses examined were Plano-T and Plano-B4 therapeutic contact lenses and Breath-O refractive lens .
	manualset3
166014	2	412552	7	NULL	NULL	0	NULL	Plano-T therapeutic contact lenses	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The soft contact lenses examined were Plano-T and Plano-B4 therapeutic contact lenses and Breath-O refractive lens .
	manualset3
166015	3	412552	7	NULL	NULL	0	NULL	Plano-B4 therapeutic contact lenses	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The soft contact lenses examined were Plano-T and Plano-B4 therapeutic contact lenses and Breath-O refractive lens .
	manualset3
166016	4	412552	7	NULL	NULL	0	NULL	Breath-O refractive lens	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The soft contact lenses examined were Plano-T and Plano-B4 therapeutic contact lenses and Breath-O refractive lens .
	manualset3
166017	1	412553	7	NULL	NULL	NULL	NULL	soil quality	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The soil quality was comparable to the most degraded bare ground soil in an adjacent bioreserve in terms of Shannon diversity index based on the communitylevel physiological profile as well as values of soil fertility indices .
	manualset3
166019	3	412553	7	NULL	NULL	0	NULL	bare ground soil	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The soil quality was comparable to the most degraded bare ground soil in an adjacent bioreserve in terms of Shannon diversity index based on the communitylevel physiological profile as well as values of soil fertility indices .
	manualset3
166020	4	412553	7	NULL	NULL	0	NULL	bioreserve	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The soil quality was comparable to the most degraded bare ground soil in an adjacent bioreserve in terms of Shannon diversity index based on the communitylevel physiological profile as well as values of soil fertility indices .
	manualset3
166021	5	412553	7	NULL	NULL	0	NULL	Shannon diversity index	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The soil quality was comparable to the most degraded bare ground soil in an adjacent bioreserve in terms of Shannon diversity index based on the communitylevel physiological profile as well as values of soil fertility indices .
	manualset3
166022	6	412553	7	NULL	NULL	0	NULL	communitylevel 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The soil quality was comparable to the most degraded bare ground soil in an adjacent bioreserve in terms of Shannon diversity index based on the communitylevel physiological profile as well as values of soil fertility indices .
	manualset3
166023	7	412553	7	NULL	NULL	NULL	NULL	physiological profile	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The soil quality was comparable to the most degraded bare ground soil in an adjacent bioreserve in terms of Shannon diversity index based on the communitylevel physiological profile as well as values of soil fertility indices .
	manualset3
166024	8	412553	7	NULL	NULL	0	NULL	values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The soil quality was comparable to the most degraded bare ground soil in an adjacent bioreserve in terms of Shannon diversity index based on the communitylevel physiological profile as well as values of soil fertility indices .
	manualset3
166025	9	412553	7	NULL	NULL	0	NULL	soil fertility indices	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The soil quality was comparable to the most degraded bare ground soil in an adjacent bioreserve in terms of Shannon diversity index based on the communitylevel physiological profile as well as values of soil fertility indices .
	manualset3
166026	1	412554	7	NULL	NULL	0	NULL	solubilization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The solubilization and partial purification of the beta-N-acetylglucosaminidase activity is reported .
	manualset3
166027	2	412554	7	NULL	NULL	0	NULL	partial purification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The solubilization and partial purification of the beta-N-acetylglucosaminidase activity is reported .
	manualset3
166028	3	412554	7	NULL	NULL	0	NULL	beta-N-acetylglucosaminidase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The solubilization and partial purification of the beta-N-acetylglucosaminidase activity is reported .
	manualset3
166029	1	412555	7	NULL	NULL	0	NULL	soluble serotonin-binding proteins ( SBP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The soluble serotonin-binding proteins ( SBP ) present in bovine frontal cortex are very similar to those reported in rat brain .
	manualset3
166030	2	412555	7	NULL	NULL	0	NULL	bovine frontal cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The soluble serotonin-binding proteins ( SBP ) present in bovine frontal cortex are very similar to those reported in rat brain .
	manualset3
166032	4	412555	7	NULL	NULL	0	NULL	rat brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The soluble serotonin-binding proteins ( SBP ) present in bovine frontal cortex are very similar to those reported in rat brain .
	manualset3
166033	1	412556	7	NULL	NULL	0	NULL	solution	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The solution of the differential equations describing the kinetic processes showed that the oxidation and the reduction of the copper ion by H2O2 are first-order with respect to the copper ion itself only when these processes approach the steady-state .
	manualset3
166034	2	412556	7	NULL	NULL	0	NULL	differential equations	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The solution of the differential equations describing the kinetic processes showed that the oxidation and the reduction of the copper ion by H2O2 are first-order with respect to the copper ion itself only when these processes approach the steady-state .
	manualset3
166035	3	412556	7	NULL	NULL	0	NULL	kinetic processes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The solution of the differential equations describing the kinetic processes showed that the oxidation and the reduction of the copper ion by H2O2 are first-order with respect to the copper ion itself only when these processes approach the steady-state .
	manualset3
166036	4	412556	7	NULL	NULL	0	NULL	oxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The solution of the differential equations describing the kinetic processes showed that the oxidation and the reduction of the copper ion by H2O2 are first-order with respect to the copper ion itself only when these processes approach the steady-state .
	manualset3
166037	5	412556	7	NULL	NULL	0	NULL	reduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The solution of the differential equations describing the kinetic processes showed that the oxidation and the reduction of the copper ion by H2O2 are first-order with respect to the copper ion itself only when these processes approach the steady-state .
	manualset3
166038	6	412556	7	NULL	NULL	0	NULL	copper ion 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The solution of the differential equations describing the kinetic processes showed that the oxidation and the reduction of the copper ion by H2O2 are first-order with respect to the copper ion itself only when these processes approach the steady-state .
	manualset3
166039	7	412556	7	NULL	NULL	0	NULL	H2O2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The solution of the differential equations describing the kinetic processes showed that the oxidation and the reduction of the copper ion by H2O2 are first-order with respect to the copper ion itself only when these processes approach the steady-state .
	manualset3
166040	8	412556	7	NULL	NULL	0	NULL	first-order	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The solution of the differential equations describing the kinetic processes showed that the oxidation and the reduction of the copper ion by H2O2 are first-order with respect to the copper ion itself only when these processes approach the steady-state .
	manualset3
166041	9	412556	7	NULL	NULL	0	NULL	 copper ion 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The solution of the differential equations describing the kinetic processes showed that the oxidation and the reduction of the copper ion by H2O2 are first-order with respect to the copper ion itself only when these processes approach the steady-state .
	manualset3
166042	10	412556	7	NULL	NULL	0	NULL	 processes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The solution of the differential equations describing the kinetic processes showed that the oxidation and the reduction of the copper ion by H2O2 are first-order with respect to the copper ion itself only when these processes approach the steady-state .
	manualset3
166043	11	412556	7	NULL	NULL	0	NULL	steady-state	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The solution of the differential equations describing the kinetic processes showed that the oxidation and the reduction of the copper ion by H2O2 are first-order with respect to the copper ion itself only when these processes approach the steady-state .
	manualset3
166044	1	412557	7	NULL	NULL	0	NULL	accuracy	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , based on its accuracy in predicting liver fibrosis , TE could be used to identify those CD patients suitable for liver biopsy .
	manualset3
166045	2	412557	7	NULL	NULL	0	NULL	liver fibrosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , based on its accuracy in predicting liver fibrosis , TE could be used to identify those CD patients suitable for liver biopsy .
	manualset3
166046	3	412557	7	NULL	NULL	NULL	NULL	 TE	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Accordingly , based on its accuracy in predicting liver fibrosis , TE could be used to identify those CD patients suitable for liver biopsy .
	manualset3
166047	4	412557	7	NULL	NULL	0	NULL	CD patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , based on its accuracy in predicting liver fibrosis , TE could be used to identify those CD patients suitable for liver biopsy .
	manualset3
166048	5	412557	7	NULL	NULL	0	NULL	 liver biopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , based on its accuracy in predicting liver fibrosis , TE could be used to identify those CD patients suitable for liver biopsy .
	manualset3
166049	1	412558	7	NULL	NULL	0	NULL	solvent effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The solvent effect of ionic liquids on the decarboxylation of 1 , 3-dimethylorotic acid and its analog in ionic was investigated .
	manualset3
166050	2	412558	7	NULL	NULL	NULL	NULL	ionic liquids	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The solvent effect of ionic liquids on the decarboxylation of 1 , 3-dimethylorotic acid and its analog in ionic was investigated .
	manualset3
166051	3	412558	7	NULL	NULL	0	NULL	decarboxylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The solvent effect of ionic liquids on the decarboxylation of 1 , 3-dimethylorotic acid and its analog in ionic was investigated .
	manualset3
166052	4	412558	7	NULL	NULL	0	NULL	1 , 3-dimethylorotic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The solvent effect of ionic liquids on the decarboxylation of 1 , 3-dimethylorotic acid and its analog in ionic was investigated .
	manualset3
166053	5	412558	7	NULL	NULL	0	NULL	analog	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The solvent effect of ionic liquids on the decarboxylation of 1 , 3-dimethylorotic acid and its analog in ionic was investigated .
	manualset3
167781	6	412558	7	NULL	NULL	0	NULL	ionic	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The solvent effect of ionic liquids on the decarboxylation of 1 , 3-dimethylorotic acid and its analog in ionic was investigated .
	manualset3
166054	1	412559	7	NULL	NULL	0	NULL	 source	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The source was an employee who contracted pertussis via a family contact .
	manualset3
166055	2	412559	7	NULL	NULL	0	NULL	employee	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The source was an employee who contracted pertussis via a family contact .
	manualset3
166056	3	412559	7	NULL	NULL	0	NULL	pertussis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The source was an employee who contracted pertussis via a family contact .
	manualset3
166057	4	412559	7	NULL	NULL	0	NULL	family contact	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The source was an employee who contracted pertussis via a family contact .
	manualset3
166058	1	412560	7	NULL	NULL	0	NULL	sow herd	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The sow herd supplying pigs to the unit was known to be free of the major swine diseases such as swine influenza , mycoplasma pneumonia , porcine reproductive and respiratory syndrome ( PRRS ) , necroproliferative enteritis , and ascarids .
	manualset3
166059	2	412560	7	NULL	NULL	0	NULL	pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The sow herd supplying pigs to the unit was known to be free of the major swine diseases such as swine influenza , mycoplasma pneumonia , porcine reproductive and respiratory syndrome ( PRRS ) , necroproliferative enteritis , and ascarids .
	manualset3
166060	3	412560	7	NULL	NULL	0	NULL	 unit	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The sow herd supplying pigs to the unit was known to be free of the major swine diseases such as swine influenza , mycoplasma pneumonia , porcine reproductive and respiratory syndrome ( PRRS ) , necroproliferative enteritis , and ascarids .
	manualset3
166061	4	412560	7	NULL	NULL	0	NULL	major swine diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The sow herd supplying pigs to the unit was known to be free of the major swine diseases such as swine influenza , mycoplasma pneumonia , porcine reproductive and respiratory syndrome ( PRRS ) , necroproliferative enteritis , and ascarids .
	manualset3
166062	5	412560	7	NULL	NULL	0	NULL	swine influenza	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The sow herd supplying pigs to the unit was known to be free of the major swine diseases such as swine influenza , mycoplasma pneumonia , porcine reproductive and respiratory syndrome ( PRRS ) , necroproliferative enteritis , and ascarids .
	manualset3
166063	6	412560	7	NULL	NULL	0	NULL	mycoplasma pneumonia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The sow herd supplying pigs to the unit was known to be free of the major swine diseases such as swine influenza , mycoplasma pneumonia , porcine reproductive and respiratory syndrome ( PRRS ) , necroproliferative enteritis , and ascarids .
	manualset3
166064	7	412560	7	NULL	NULL	0	NULL	porcine reproductive syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The sow herd supplying pigs to the unit was known to be free of the major swine diseases such as swine influenza , mycoplasma pneumonia , porcine reproductive and respiratory syndrome ( PRRS ) , necroproliferative enteritis , and ascarids .
	manualset3
166065	8	412560	7	NULL	NULL	0	NULL	respiratory syndrome ( PRRS )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The sow herd supplying pigs to the unit was known to be free of the major swine diseases such as swine influenza , mycoplasma pneumonia , porcine reproductive and respiratory syndrome ( PRRS ) , necroproliferative enteritis , and ascarids .
	manualset3
166066	9	412560	7	NULL	NULL	0	NULL	necroproliferative enteritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The sow herd supplying pigs to the unit was known to be free of the major swine diseases such as swine influenza , mycoplasma pneumonia , porcine reproductive and respiratory syndrome ( PRRS ) , necroproliferative enteritis , and ascarids .
	manualset3
166067	10	412560	7	NULL	NULL	0	NULL	ascarids	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The sow herd supplying pigs to the unit was known to be free of the major swine diseases such as swine influenza , mycoplasma pneumonia , porcine reproductive and respiratory syndrome ( PRRS ) , necroproliferative enteritis , and ascarids .
	manualset3
166068	1	412561	7	NULL	NULL	0	NULL	spatial distribution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The spatial distribution of GmODC and GmADC transcripts in primary and lateral roots and hypocotyls revealed that these genes are co-expressed in expanding cells of cortex parenchyma , expanding cells of central cylinder in main roots and in developing tissues and expanding cells of soybean hypocotyls .
	manualset3
166069	2	412561	7	NULL	NULL	0	NULL	GmODC transcript	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The spatial distribution of GmODC and GmADC transcripts in primary and lateral roots and hypocotyls revealed that these genes are co-expressed in expanding cells of cortex parenchyma , expanding cells of central cylinder in main roots and in developing tissues and expanding cells of soybean hypocotyls .
	manualset3
166070	3	412561	7	NULL	NULL	0	NULL	GmADC transcript	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The spatial distribution of GmODC and GmADC transcripts in primary and lateral roots and hypocotyls revealed that these genes are co-expressed in expanding cells of cortex parenchyma , expanding cells of central cylinder in main roots and in developing tissues and expanding cells of soybean hypocotyls .
	manualset3
166071	4	412561	7	NULL	NULL	0	NULL	primary roots	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The spatial distribution of GmODC and GmADC transcripts in primary and lateral roots and hypocotyls revealed that these genes are co-expressed in expanding cells of cortex parenchyma , expanding cells of central cylinder in main roots and in developing tissues and expanding cells of soybean hypocotyls .
	manualset3
166072	5	412561	7	NULL	NULL	0	NULL	 lateral roots	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The spatial distribution of GmODC and GmADC transcripts in primary and lateral roots and hypocotyls revealed that these genes are co-expressed in expanding cells of cortex parenchyma , expanding cells of central cylinder in main roots and in developing tissues and expanding cells of soybean hypocotyls .
	manualset3
166073	6	412561	7	NULL	NULL	0	NULL	hypocotyls	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The spatial distribution of GmODC and GmADC transcripts in primary and lateral roots and hypocotyls revealed that these genes are co-expressed in expanding cells of cortex parenchyma , expanding cells of central cylinder in main roots and in developing tissues and expanding cells of soybean hypocotyls .
	manualset3
166074	7	412561	7	NULL	NULL	0	NULL	 genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The spatial distribution of GmODC and GmADC transcripts in primary and lateral roots and hypocotyls revealed that these genes are co-expressed in expanding cells of cortex parenchyma , expanding cells of central cylinder in main roots and in developing tissues and expanding cells of soybean hypocotyls .
	manualset3
166075	8	412561	7	NULL	NULL	0	NULL	expanding cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The spatial distribution of GmODC and GmADC transcripts in primary and lateral roots and hypocotyls revealed that these genes are co-expressed in expanding cells of cortex parenchyma , expanding cells of central cylinder in main roots and in developing tissues and expanding cells of soybean hypocotyls .
	manualset3
166076	9	412561	7	NULL	NULL	0	NULL	cortex parenchyma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The spatial distribution of GmODC and GmADC transcripts in primary and lateral roots and hypocotyls revealed that these genes are co-expressed in expanding cells of cortex parenchyma , expanding cells of central cylinder in main roots and in developing tissues and expanding cells of soybean hypocotyls .
	manualset3
166077	10	412561	7	NULL	NULL	0	NULL	expanding cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The spatial distribution of GmODC and GmADC transcripts in primary and lateral roots and hypocotyls revealed that these genes are co-expressed in expanding cells of cortex parenchyma , expanding cells of central cylinder in main roots and in developing tissues and expanding cells of soybean hypocotyls .
	manualset3
166078	11	412561	7	NULL	NULL	0	NULL	central cylinder	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The spatial distribution of GmODC and GmADC transcripts in primary and lateral roots and hypocotyls revealed that these genes are co-expressed in expanding cells of cortex parenchyma , expanding cells of central cylinder in main roots and in developing tissues and expanding cells of soybean hypocotyls .
	manualset3
166079	12	412561	7	NULL	NULL	0	NULL	main roots 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The spatial distribution of GmODC and GmADC transcripts in primary and lateral roots and hypocotyls revealed that these genes are co-expressed in expanding cells of cortex parenchyma , expanding cells of central cylinder in main roots and in developing tissues and expanding cells of soybean hypocotyls .
	manualset3
166080	13	412561	7	NULL	NULL	0	NULL	tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The spatial distribution of GmODC and GmADC transcripts in primary and lateral roots and hypocotyls revealed that these genes are co-expressed in expanding cells of cortex parenchyma , expanding cells of central cylinder in main roots and in developing tissues and expanding cells of soybean hypocotyls .
	manualset3
166081	14	412561	7	NULL	NULL	0	NULL	expanding cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The spatial distribution of GmODC and GmADC transcripts in primary and lateral roots and hypocotyls revealed that these genes are co-expressed in expanding cells of cortex parenchyma , expanding cells of central cylinder in main roots and in developing tissues and expanding cells of soybean hypocotyls .
	manualset3
166082	15	412561	7	NULL	NULL	0	NULL	soybean hypocotyls	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The spatial distribution of GmODC and GmADC transcripts in primary and lateral roots and hypocotyls revealed that these genes are co-expressed in expanding cells of cortex parenchyma , expanding cells of central cylinder in main roots and in developing tissues and expanding cells of soybean hypocotyls .
	manualset3
166083	1	412562	7	NULL	NULL	0	NULL	spatial scale	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The spatial scale on which microbial communities respond to plant invasions may provide important clues as to the nature of potential invader-microbe interactions .
	manualset3
166084	2	412562	7	NULL	NULL	0	NULL	microbial communities	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The spatial scale on which microbial communities respond to plant invasions may provide important clues as to the nature of potential invader-microbe interactions .
	manualset3
166085	3	412562	7	NULL	NULL	0	NULL	plant invasions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The spatial scale on which microbial communities respond to plant invasions may provide important clues as to the nature of potential invader-microbe interactions .
	manualset3
166086	4	412562	7	NULL	NULL	0	NULL	nature	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The spatial scale on which microbial communities respond to plant invasions may provide important clues as to the nature of potential invader-microbe interactions .
	manualset3
166087	5	412562	7	NULL	NULL	0	NULL	invader-microbe interactions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The spatial scale on which microbial communities respond to plant invasions may provide important clues as to the nature of potential invader-microbe interactions .
	manualset3
166088	1	412563	7	NULL	NULL	0	NULL	special forms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The special forms , the rudiment , triphalangism , and multiple duplication , can easily be further subclassified .
	manualset3
166089	2	412563	7	NULL	NULL	0	NULL	rudiment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The special forms , the rudiment , triphalangism , and multiple duplication , can easily be further subclassified .
	manualset3
166090	3	412563	7	NULL	NULL	0	NULL	triphalangism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The special forms , the rudiment , triphalangism , and multiple duplication , can easily be further subclassified .
	manualset3
166091	4	412563	7	NULL	NULL	0	NULL	multiple duplication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The special forms , the rudiment , triphalangism , and multiple duplication , can easily be further subclassified .
	manualset3
166092	1	412564	7	NULL	NULL	0	NULL	lower bite plate	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The specially designed lower bite plate is dynamic and allows for both rotation and translation of the lower jaw during movement , thus , permitting the natural curvilinear trajectory of the jaw .
	manualset3
166094	3	412564	7	NULL	NULL	0	NULL	 rotation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The specially designed lower bite plate is dynamic and allows for both rotation and translation of the lower jaw during movement , thus , permitting the natural curvilinear trajectory of the jaw .
	manualset3
166095	4	412564	7	NULL	NULL	0	NULL	 translation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The specially designed lower bite plate is dynamic and allows for both rotation and translation of the lower jaw during movement , thus , permitting the natural curvilinear trajectory of the jaw .
	manualset3
166096	5	412564	7	NULL	NULL	0	NULL	 lower jaw	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The specially designed lower bite plate is dynamic and allows for both rotation and translation of the lower jaw during movement , thus , permitting the natural curvilinear trajectory of the jaw .
	manualset3
166097	6	412564	7	NULL	NULL	0	NULL	movement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The specially designed lower bite plate is dynamic and allows for both rotation and translation of the lower jaw during movement , thus , permitting the natural curvilinear trajectory of the jaw .
	manualset3
166098	7	412564	7	NULL	NULL	0	NULL	 natural curvilinear trajectory 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The specially designed lower bite plate is dynamic and allows for both rotation and translation of the lower jaw during movement , thus , permitting the natural curvilinear trajectory of the jaw .
	manualset3
166099	8	412564	7	NULL	NULL	0	NULL	jaw	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The specially designed lower bite plate is dynamic and allows for both rotation and translation of the lower jaw during movement , thus , permitting the natural curvilinear trajectory of the jaw .
	manualset3
166100	1	412565	7	NULL	NULL	0	NULL	baseline proliferating cell nuclear antigen levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , baseline proliferating cell nuclear antigen levels are lower in Pbx1 ( + / - ) mice , and unilateral adrenalectomy results in impaired contralateral compensatory adrenal growth , indicating a lower proliferative potential in the context of Pbx1 haploinsufficiency .
	manualset3
166101	2	412565	7	NULL	NULL	0	NULL	Pbx1 ( + / - ) mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , baseline proliferating cell nuclear antigen levels are lower in Pbx1 ( + / - ) mice , and unilateral adrenalectomy results in impaired contralateral compensatory adrenal growth , indicating a lower proliferative potential in the context of Pbx1 haploinsufficiency .
	manualset3
166102	3	412565	7	NULL	NULL	0	NULL	unilateral adrenalectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , baseline proliferating cell nuclear antigen levels are lower in Pbx1 ( + / - ) mice , and unilateral adrenalectomy results in impaired contralateral compensatory adrenal growth , indicating a lower proliferative potential in the context of Pbx1 haploinsufficiency .
	manualset3
166103	4	412565	7	NULL	NULL	0	NULL	impaired contralateral compensatory adrenal growth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , baseline proliferating cell nuclear antigen levels are lower in Pbx1 ( + / - ) mice , and unilateral adrenalectomy results in impaired contralateral compensatory adrenal growth , indicating a lower proliferative potential in the context of Pbx1 haploinsufficiency .
	manualset3
166104	5	412565	7	NULL	NULL	0	NULL	lower proliferative potential 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , baseline proliferating cell nuclear antigen levels are lower in Pbx1 ( + / - ) mice , and unilateral adrenalectomy results in impaired contralateral compensatory adrenal growth , indicating a lower proliferative potential in the context of Pbx1 haploinsufficiency .
	manualset3
166105	6	412565	7	NULL	NULL	0	NULL	context 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , baseline proliferating cell nuclear antigen levels are lower in Pbx1 ( + / - ) mice , and unilateral adrenalectomy results in impaired contralateral compensatory adrenal growth , indicating a lower proliferative potential in the context of Pbx1 haploinsufficiency .
	manualset3
166106	7	412565	7	NULL	NULL	0	NULL	Pbx1 haploinsufficiency 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , baseline proliferating cell nuclear antigen levels are lower in Pbx1 ( + / - ) mice , and unilateral adrenalectomy results in impaired contralateral compensatory adrenal growth , indicating a lower proliferative potential in the context of Pbx1 haploinsufficiency .
	manualset3
166107	1	412566	7	NULL	NULL	0	NULL	species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The species that decreased in abundance have functional traits linked to seagrass habitats that regressed consecutively to increasing eutrophication .
	manualset3
166108	2	412566	7	NULL	NULL	0	NULL	functional traits	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The species that decreased in abundance have functional traits linked to seagrass habitats that regressed consecutively to increasing eutrophication .
	manualset3
166109	3	412566	7	NULL	NULL	0	NULL	seagrass habitats	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The species that decreased in abundance have functional traits linked to seagrass habitats that regressed consecutively to increasing eutrophication .
	manualset3
166110	4	412566	7	NULL	NULL	NULL	NULL	eutrophication	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The species that decreased in abundance have functional traits linked to seagrass habitats that regressed consecutively to increasing eutrophication .
	manualset3
166111	5	412566	7	NULL	NULL	0	NULL	abundance	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The species that decreased in abundance have functional traits linked to seagrass habitats that regressed consecutively to increasing eutrophication .
	manualset3
166112	1	412567	7	NULL	NULL	0	NULL	CXCR4 inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The specific CXCR4 inhibitor AMD3100 and the anti-CXCR4 antibody MAB171 inhibited the migration of MM cells in vitro .
	manualset3
166113	2	412567	7	NULL	NULL	0	NULL	AMD3100	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The specific CXCR4 inhibitor AMD3100 and the anti-CXCR4 antibody MAB171 inhibited the migration of MM cells in vitro .
	manualset3
166114	3	412567	7	NULL	NULL	0	NULL	anti-CXCR4 antibody MAB171	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The specific CXCR4 inhibitor AMD3100 and the anti-CXCR4 antibody MAB171 inhibited the migration of MM cells in vitro .
	manualset3
166115	4	412567	7	NULL	NULL	0	NULL	migration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The specific CXCR4 inhibitor AMD3100 and the anti-CXCR4 antibody MAB171 inhibited the migration of MM cells in vitro .
	manualset3
166116	5	412567	7	NULL	NULL	0	NULL	MM cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The specific CXCR4 inhibitor AMD3100 and the anti-CXCR4 antibody MAB171 inhibited the migration of MM cells in vitro .
	manualset3
166117	1	412568	7	NULL	NULL	0	NULL	specific activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The specific activity is 43 U/mg at 25 degrees C in the presence of Mn2 + ions and 31 U/mg under previously reported conditions and assuming a specific absorption coefficient of 1.29 cm2/mg at 280 nm .
	manualset3
166118	2	412568	7	NULL	NULL	0	NULL	 43 U/mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The specific activity is 43 U/mg at 25 degrees C in the presence of Mn2 + ions and 31 U/mg under previously reported conditions and assuming a specific absorption coefficient of 1.29 cm2/mg at 280 nm .
	manualset3
166119	3	412568	7	NULL	NULL	0	NULL	25 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The specific activity is 43 U/mg at 25 degrees C in the presence of Mn2 + ions and 31 U/mg under previously reported conditions and assuming a specific absorption coefficient of 1.29 cm2/mg at 280 nm .
	manualset3
166120	4	412568	7	NULL	NULL	0	NULL	Mn2 + ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The specific activity is 43 U/mg at 25 degrees C in the presence of Mn2 + ions and 31 U/mg under previously reported conditions and assuming a specific absorption coefficient of 1.29 cm2/mg at 280 nm .
	manualset3
166121	5	412568	7	NULL	NULL	0	NULL	31 U/mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The specific activity is 43 U/mg at 25 degrees C in the presence of Mn2 + ions and 31 U/mg under previously reported conditions and assuming a specific absorption coefficient of 1.29 cm2/mg at 280 nm .
	manualset3
166122	6	412568	7	NULL	NULL	0	NULL	conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The specific activity is 43 U/mg at 25 degrees C in the presence of Mn2 + ions and 31 U/mg under previously reported conditions and assuming a specific absorption coefficient of 1.29 cm2/mg at 280 nm .
	manualset3
166123	7	412568	7	NULL	NULL	0	NULL	specific absorption coefficient	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The specific activity is 43 U/mg at 25 degrees C in the presence of Mn2 + ions and 31 U/mg under previously reported conditions and assuming a specific absorption coefficient of 1.29 cm2/mg at 280 nm .
	manualset3
166124	8	412568	7	NULL	NULL	0	NULL	1.29 cm2/mg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The specific activity is 43 U/mg at 25 degrees C in the presence of Mn2 + ions and 31 U/mg under previously reported conditions and assuming a specific absorption coefficient of 1.29 cm2/mg at 280 nm .
	manualset3
166125	9	412568	7	NULL	NULL	0	NULL	280 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The specific activity is 43 U/mg at 25 degrees C in the presence of Mn2 + ions and 31 U/mg under previously reported conditions and assuming a specific absorption coefficient of 1.29 cm2/mg at 280 nm .
	manualset3
166126	1	412569	7	NULL	NULL	0	NULL	specific cell sources	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The specific cell sources and signals for induction of various colony-stimulating factors ( CSF ) in peripheral blood mononuclear cells ( PBMC ) , purified T lymphocyte and monocyte ( Mo ) populations have been investigated .
	manualset3
166127	2	412569	7	NULL	NULL	0	NULL	signals 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The specific cell sources and signals for induction of various colony-stimulating factors ( CSF ) in peripheral blood mononuclear cells ( PBMC ) , purified T lymphocyte and monocyte ( Mo ) populations have been investigated .
	manualset3
166128	3	412569	7	NULL	NULL	0	NULL	induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The specific cell sources and signals for induction of various colony-stimulating factors ( CSF ) in peripheral blood mononuclear cells ( PBMC ) , purified T lymphocyte and monocyte ( Mo ) populations have been investigated .
	manualset3
166129	4	412569	7	NULL	NULL	0	NULL	colony-stimulating factors ( CSF )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The specific cell sources and signals for induction of various colony-stimulating factors ( CSF ) in peripheral blood mononuclear cells ( PBMC ) , purified T lymphocyte and monocyte ( Mo ) populations have been investigated .
	manualset3
166130	5	412569	7	NULL	NULL	0	NULL	peripheral blood mononuclear cells ( PBMC )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The specific cell sources and signals for induction of various colony-stimulating factors ( CSF ) in peripheral blood mononuclear cells ( PBMC ) , purified T lymphocyte and monocyte ( Mo ) populations have been investigated .
	manualset3
166131	6	412569	7	NULL	NULL	0	NULL	purified T lymphocyte populations	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The specific cell sources and signals for induction of various colony-stimulating factors ( CSF ) in peripheral blood mononuclear cells ( PBMC ) , purified T lymphocyte and monocyte ( Mo ) populations have been investigated .
	manualset3
166132	7	412569	7	NULL	NULL	0	NULL	monocyte ( Mo ) populations	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The specific cell sources and signals for induction of various colony-stimulating factors ( CSF ) in peripheral blood mononuclear cells ( PBMC ) , purified T lymphocyte and monocyte ( Mo ) populations have been investigated .
	manualset3
166133	1	412570	7	NULL	NULL	0	NULL	specific constellation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The specific constellation of symptoms that will manifest in the effected individual depends on the type of genetic defect in the mitochondria .
	manualset3
166134	2	412570	7	NULL	NULL	0	NULL	symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The specific constellation of symptoms that will manifest in the effected individual depends on the type of genetic defect in the mitochondria .
	manualset3
166135	3	412570	7	NULL	NULL	0	NULL	individual	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The specific constellation of symptoms that will manifest in the effected individual depends on the type of genetic defect in the mitochondria .
	manualset3
166136	4	412570	7	NULL	NULL	0	NULL	type	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The specific constellation of symptoms that will manifest in the effected individual depends on the type of genetic defect in the mitochondria .
	manualset3
166137	5	412570	7	NULL	NULL	0	NULL	genetic defect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The specific constellation of symptoms that will manifest in the effected individual depends on the type of genetic defect in the mitochondria .
	manualset3
166138	6	412570	7	NULL	NULL	0	NULL	mitochondria	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The specific constellation of symptoms that will manifest in the effected individual depends on the type of genetic defect in the mitochondria .
	manualset3
166139	1	412571	7	NULL	NULL	0	NULL	specific step	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The specific step in fertilization which is dysfunctional , however , is not known .
	manualset3
166140	2	412571	7	NULL	NULL	0	NULL	fertilization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The specific step in fertilization which is dysfunctional , however , is not known .
	manualset3
166142	1	412572	7	NULL	NULL	0	NULL	context	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , in the context of a high-risk population ( The Bahamas ) for HIV , a 17-item scale -- the Condom-use Skills Checklist ( CUSC ) -- was developed for use among young adolescents and adults .
	manualset3
166143	2	412572	7	NULL	NULL	0	NULL	high-risk population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , in the context of a high-risk population ( The Bahamas ) for HIV , a 17-item scale -- the Condom-use Skills Checklist ( CUSC ) -- was developed for use among young adolescents and adults .
	manualset3
166144	3	412572	7	NULL	NULL	0	NULL	The Bahamas	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , in the context of a high-risk population ( The Bahamas ) for HIV , a 17-item scale -- the Condom-use Skills Checklist ( CUSC ) -- was developed for use among young adolescents and adults .
	manualset3
166145	4	412572	7	NULL	NULL	0	NULL	HIV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , in the context of a high-risk population ( The Bahamas ) for HIV , a 17-item scale -- the Condom-use Skills Checklist ( CUSC ) -- was developed for use among young adolescents and adults .
	manualset3
166146	5	412572	7	NULL	NULL	0	NULL	17-item scale	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , in the context of a high-risk population ( The Bahamas ) for HIV , a 17-item scale -- the Condom-use Skills Checklist ( CUSC ) -- was developed for use among young adolescents and adults .
	manualset3
166147	6	412572	7	NULL	NULL	0	NULL	Condom-use Skills Checklist ( CUSC )	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , in the context of a high-risk population ( The Bahamas ) for HIV , a 17-item scale -- the Condom-use Skills Checklist ( CUSC ) -- was developed for use among young adolescents and adults .
	manualset3
166148	7	412572	7	NULL	NULL	0	NULL	young adolescents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , in the context of a high-risk population ( The Bahamas ) for HIV , a 17-item scale -- the Condom-use Skills Checklist ( CUSC ) -- was developed for use among young adolescents and adults .
	manualset3
166149	8	412572	7	NULL	NULL	0	NULL	adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , in the context of a high-risk population ( The Bahamas ) for HIV , a 17-item scale -- the Condom-use Skills Checklist ( CUSC ) -- was developed for use among young adolescents and adults .
	manualset3
166150	1	412573	7	NULL	NULL	0	NULL	specificity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The specificity and pattern of Es-vasa expression in gonads indicates that it may be used as molecular marker for germ line in E. sinensis .
	manualset3
166151	2	412573	7	NULL	NULL	0	NULL	 pattern	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The specificity and pattern of Es-vasa expression in gonads indicates that it may be used as molecular marker for germ line in E. sinensis .
	manualset3
166152	3	412573	7	NULL	NULL	0	NULL	Es-vasa expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The specificity and pattern of Es-vasa expression in gonads indicates that it may be used as molecular marker for germ line in E. sinensis .
	manualset3
166153	4	412573	7	NULL	NULL	0	NULL	gonads	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The specificity and pattern of Es-vasa expression in gonads indicates that it may be used as molecular marker for germ line in E. sinensis .
	manualset3
166154	5	412573	7	NULL	NULL	0	NULL	molecular marker	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The specificity and pattern of Es-vasa expression in gonads indicates that it may be used as molecular marker for germ line in E. sinensis .
	manualset3
166155	6	412573	7	NULL	NULL	0	NULL	germ line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The specificity and pattern of Es-vasa expression in gonads indicates that it may be used as molecular marker for germ line in E. sinensis .
	manualset3
166156	7	412573	7	NULL	NULL	0	NULL	E. sinensis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The specificity and pattern of Es-vasa expression in gonads indicates that it may be used as molecular marker for germ line in E. sinensis .
	manualset3
166157	1	412574	7	NULL	NULL	0	NULL	specificity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The specificity of a monoclonal antibody RIA for the measurement of free alpha-subunit in plasma is presently documented .
	manualset3
166158	2	412574	7	NULL	NULL	0	NULL	monoclonal antibody RIA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The specificity of a monoclonal antibody RIA for the measurement of free alpha-subunit in plasma is presently documented .
	manualset3
166159	3	412574	7	NULL	NULL	0	NULL	measurement	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The specificity of a monoclonal antibody RIA for the measurement of free alpha-subunit in plasma is presently documented .
	manualset3
166160	4	412574	7	NULL	NULL	0	NULL	free alpha-subunit	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The specificity of a monoclonal antibody RIA for the measurement of free alpha-subunit in plasma is presently documented .
	manualset3
166161	5	412574	7	NULL	NULL	0	NULL	plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The specificity of a monoclonal antibody RIA for the measurement of free alpha-subunit in plasma is presently documented .
	manualset3
166162	1	412575	7	NULL	NULL	0	NULL	specificity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The specificity of mathematical modeling of optimal dose fields in radiation therapy of malignant tumors is under consideration .
	manualset3
166163	2	412575	7	NULL	NULL	0	NULL	mathematical modeling	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The specificity of mathematical modeling of optimal dose fields in radiation therapy of malignant tumors is under consideration .
	manualset3
166164	3	412575	7	NULL	NULL	0	NULL	optimal dose fields	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The specificity of mathematical modeling of optimal dose fields in radiation therapy of malignant tumors is under consideration .
	manualset3
166165	4	412575	7	NULL	NULL	0	NULL	radiation therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The specificity of mathematical modeling of optimal dose fields in radiation therapy of malignant tumors is under consideration .
	manualset3
166166	5	412575	7	NULL	NULL	0	NULL	malignant tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The specificity of mathematical modeling of optimal dose fields in radiation therapy of malignant tumors is under consideration .
	manualset3
166167	6	412575	7	NULL	NULL	0	NULL	consideration	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The specificity of mathematical modeling of optimal dose fields in radiation therapy of malignant tumors is under consideration .
	manualset3
166168	1	412576	7	NULL	NULL	0	NULL	specificity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The specificity of the assay was confirmed using a panel of viral and bacterial pathogens of poultry .
	manualset3
166169	2	412576	7	NULL	NULL	0	NULL	assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The specificity of the assay was confirmed using a panel of viral and bacterial pathogens of poultry .
	manualset3
166170	3	412576	7	NULL	NULL	0	NULL	panel 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The specificity of the assay was confirmed using a panel of viral and bacterial pathogens of poultry .
	manualset3
166171	4	412576	7	NULL	NULL	0	NULL	viral pathogens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The specificity of the assay was confirmed using a panel of viral and bacterial pathogens of poultry .
	manualset3
166172	5	412576	7	NULL	NULL	0	NULL	 bacterial pathogens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The specificity of the assay was confirmed using a panel of viral and bacterial pathogens of poultry .
	manualset3
166173	6	412576	7	NULL	NULL	0	NULL	poultry	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The specificity of the assay was confirmed using a panel of viral and bacterial pathogens of poultry .
	manualset3
166174	1	412577	7	NULL	NULL	0	NULL	specimens	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The specimens of kidneys were used for pathological examination ( hematoxylin-eosin staining ) , detection of alpha-SMA and TGF-beta1 mRNA ( Reverse transcriptase-polymerase chain reaction ) and protein ( Western blot and immunohistochemistry ) expression .
	manualset3
166175	2	412577	7	NULL	NULL	0	NULL	kidneys	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The specimens of kidneys were used for pathological examination ( hematoxylin-eosin staining ) , detection of alpha-SMA and TGF-beta1 mRNA ( Reverse transcriptase-polymerase chain reaction ) and protein ( Western blot and immunohistochemistry ) expression .
	manualset3
166176	3	412577	7	NULL	NULL	0	NULL	pathological examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The specimens of kidneys were used for pathological examination ( hematoxylin-eosin staining ) , detection of alpha-SMA and TGF-beta1 mRNA ( Reverse transcriptase-polymerase chain reaction ) and protein ( Western blot and immunohistochemistry ) expression .
	manualset3
166177	4	412577	7	NULL	NULL	0	NULL	hematoxylin-eosin staining	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The specimens of kidneys were used for pathological examination ( hematoxylin-eosin staining ) , detection of alpha-SMA and TGF-beta1 mRNA ( Reverse transcriptase-polymerase chain reaction ) and protein ( Western blot and immunohistochemistry ) expression .
	manualset3
166178	5	412577	7	NULL	NULL	0	NULL	detection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The specimens of kidneys were used for pathological examination ( hematoxylin-eosin staining ) , detection of alpha-SMA and TGF-beta1 mRNA ( Reverse transcriptase-polymerase chain reaction ) and protein ( Western blot and immunohistochemistry ) expression .
	manualset3
166179	6	412577	7	NULL	NULL	0	NULL	alpha-SMA mRNA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The specimens of kidneys were used for pathological examination ( hematoxylin-eosin staining ) , detection of alpha-SMA and TGF-beta1 mRNA ( Reverse transcriptase-polymerase chain reaction ) and protein ( Western blot and immunohistochemistry ) expression .
	manualset3
166180	7	412577	7	NULL	NULL	0	NULL	TGF-beta1 mRNA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The specimens of kidneys were used for pathological examination ( hematoxylin-eosin staining ) , detection of alpha-SMA and TGF-beta1 mRNA ( Reverse transcriptase-polymerase chain reaction ) and protein ( Western blot and immunohistochemistry ) expression .
	manualset3
166181	8	412577	7	NULL	NULL	0	NULL	Reverse transcriptase-polymerase chain reaction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The specimens of kidneys were used for pathological examination ( hematoxylin-eosin staining ) , detection of alpha-SMA and TGF-beta1 mRNA ( Reverse transcriptase-polymerase chain reaction ) and protein ( Western blot and immunohistochemistry ) expression .
	manualset3
166182	9	412577	7	NULL	NULL	0	NULL	protein expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The specimens of kidneys were used for pathological examination ( hematoxylin-eosin staining ) , detection of alpha-SMA and TGF-beta1 mRNA ( Reverse transcriptase-polymerase chain reaction ) and protein ( Western blot and immunohistochemistry ) expression .
	manualset3
166183	10	412577	7	NULL	NULL	0	NULL	Western blot 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The specimens of kidneys were used for pathological examination ( hematoxylin-eosin staining ) , detection of alpha-SMA and TGF-beta1 mRNA ( Reverse transcriptase-polymerase chain reaction ) and protein ( Western blot and immunohistochemistry ) expression .
	manualset3
166184	11	412577	7	NULL	NULL	0	NULL	immunohistochemistry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The specimens of kidneys were used for pathological examination ( hematoxylin-eosin staining ) , detection of alpha-SMA and TGF-beta1 mRNA ( Reverse transcriptase-polymerase chain reaction ) and protein ( Western blot and immunohistochemistry ) expression .
	manualset3
166185	1	412578	7	NULL	NULL	NULL	NULL	specimens	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The specimens were exposed at varying energy densities to a single pass of the laser .
	manualset3
166186	2	412578	7	NULL	NULL	0	NULL	energy densities	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The specimens were exposed at varying energy densities to a single pass of the laser .
	manualset3
166187	3	412578	7	NULL	NULL	0	NULL	single pass	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The specimens were exposed at varying energy densities to a single pass of the laser .
	manualset3
166188	4	412578	7	NULL	NULL	0	NULL	laser	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The specimens were exposed at varying energy densities to a single pass of the laser .
	manualset3
166189	1	412579	7	NULL	NULL	0	NULL	 specimens	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The specimens were then stored in 5 % basic fuchsin dye for 2 days .
	manualset3
166190	2	412579	7	NULL	NULL	0	NULL	5 % basic fuchsin dye	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The specimens were then stored in 5 % basic fuchsin dye for 2 days .
	manualset3
166191	3	412579	7	NULL	NULL	0	NULL	2 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The specimens were then stored in 5 % basic fuchsin dye for 2 days .
	manualset3
166192	1	412580	7	NULL	NULL	NULL	NULL	specimens 	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The specimens were then treated with one of the following etch-and-rinse adhesive systems : a 3-step , water-based system ( Adper Scotchbond Multipurpose , or SBMP ) or a 2-step , ethanol/water-based system ( Adper Single Bond 2 , or SB ) .
	manualset3
166193	2	412580	7	NULL	NULL	0	NULL	etch-and-rinse adhesive systems	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The specimens were then treated with one of the following etch-and-rinse adhesive systems : a 3-step , water-based system ( Adper Scotchbond Multipurpose , or SBMP ) or a 2-step , ethanol/water-based system ( Adper Single Bond 2 , or SB ) .
	manualset3
166194	3	412580	7	NULL	NULL	NULL	NULL	3-step  water-based system	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The specimens were then treated with one of the following etch-and-rinse adhesive systems : a 3-step , water-based system ( Adper Scotchbond Multipurpose , or SBMP ) or a 2-step , ethanol/water-based system ( Adper Single Bond 2 , or SB ) .
	manualset3
166196	5	412580	7	NULL	NULL	0	NULL	Adper Scotchbond Multipurpose	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The specimens were then treated with one of the following etch-and-rinse adhesive systems : a 3-step , water-based system ( Adper Scotchbond Multipurpose , or SBMP ) or a 2-step , ethanol/water-based system ( Adper Single Bond 2 , or SB ) .
	manualset3
166197	6	412580	7	NULL	NULL	0	NULL	SBMP 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The specimens were then treated with one of the following etch-and-rinse adhesive systems : a 3-step , water-based system ( Adper Scotchbond Multipurpose , or SBMP ) or a 2-step , ethanol/water-based system ( Adper Single Bond 2 , or SB ) .
	manualset3
166198	7	412580	7	NULL	NULL	NULL	NULL	2-step ethanol/water-based system	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The specimens were then treated with one of the following etch-and-rinse adhesive systems : a 3-step , water-based system ( Adper Scotchbond Multipurpose , or SBMP ) or a 2-step , ethanol/water-based system ( Adper Single Bond 2 , or SB ) .
	manualset3
166200	9	412580	7	NULL	NULL	0	NULL	Adper Single Bond 2	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The specimens were then treated with one of the following etch-and-rinse adhesive systems : a 3-step , water-based system ( Adper Scotchbond Multipurpose , or SBMP ) or a 2-step , ethanol/water-based system ( Adper Single Bond 2 , or SB ) .
	manualset3
166201	10	412580	7	NULL	NULL	NULL	NULL	SB	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The specimens were then treated with one of the following etch-and-rinse adhesive systems : a 3-step , water-based system ( Adper Scotchbond Multipurpose , or SBMP ) or a 2-step , ethanol/water-based system ( Adper Single Bond 2 , or SB ) .
	manualset3
166202	1	412581	7	NULL	NULL	0	NULL	Clinico-statistical note	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinico-statistical note on 2000 cesarean sections for 1954 to 1964 ) .
	manualset3
166203	2	412581	7	NULL	NULL	0	NULL	 2000	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinico-statistical note on 2000 cesarean sections for 1954 to 1964 ) .
	manualset3
166204	3	412581	7	NULL	NULL	0	NULL	cesarean sections	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinico-statistical note on 2000 cesarean sections for 1954 to 1964 ) .
	manualset3
166205	4	412581	7	NULL	NULL	0	NULL	1954 to 1964 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinico-statistical note on 2000 cesarean sections for 1954 to 1964 ) .
	manualset3
166206	1	412582	7	NULL	NULL	0	NULL	spectral amplitude change	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The spectral amplitude change induced by a large scopolamine dose could not be augmented by either mecamylamine or an additional injection of scopolamine .
	manualset3
166207	2	412582	7	NULL	NULL	0	NULL	scopolamine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The spectral amplitude change induced by a large scopolamine dose could not be augmented by either mecamylamine or an additional injection of scopolamine .
	manualset3
166208	3	412582	7	NULL	NULL	0	NULL	dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The spectral amplitude change induced by a large scopolamine dose could not be augmented by either mecamylamine or an additional injection of scopolamine .
	manualset3
166209	4	412582	7	NULL	NULL	0	NULL	mecamylamine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The spectral amplitude change induced by a large scopolamine dose could not be augmented by either mecamylamine or an additional injection of scopolamine .
	manualset3
166210	5	412582	7	NULL	NULL	0	NULL	injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The spectral amplitude change induced by a large scopolamine dose could not be augmented by either mecamylamine or an additional injection of scopolamine .
	manualset3
166211	6	412582	7	NULL	NULL	NULL	NULL	scopolamine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The spectral amplitude change induced by a large scopolamine dose could not be augmented by either mecamylamine or an additional injection of scopolamine .
	manualset3
166212	1	412583	7	NULL	NULL	NULL	NULL	spectral properties	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The spectral properties of the beta B2 mutants , as well as their stabilities against denaturants , resemble those of wild-type beta B2-crystallin , thus indicating that the overall peptide fold of the subunits is not changed significantly .
	manualset3
166213	2	412583	7	NULL	NULL	0	NULL	beta B2 mutants	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The spectral properties of the beta B2 mutants , as well as their stabilities against denaturants , resemble those of wild-type beta B2-crystallin , thus indicating that the overall peptide fold of the subunits is not changed significantly .
	manualset3
166214	3	412583	7	NULL	NULL	0	NULL	 stabilities 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The spectral properties of the beta B2 mutants , as well as their stabilities against denaturants , resemble those of wild-type beta B2-crystallin , thus indicating that the overall peptide fold of the subunits is not changed significantly .
	manualset3
166215	4	412583	7	NULL	NULL	0	NULL	denaturants	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The spectral properties of the beta B2 mutants , as well as their stabilities against denaturants , resemble those of wild-type beta B2-crystallin , thus indicating that the overall peptide fold of the subunits is not changed significantly .
	manualset3
166216	5	412583	7	NULL	NULL	0	NULL	wild-type beta B2-crystallin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The spectral properties of the beta B2 mutants , as well as their stabilities against denaturants , resemble those of wild-type beta B2-crystallin , thus indicating that the overall peptide fold of the subunits is not changed significantly .
	manualset3
166217	6	412583	7	NULL	NULL	0	NULL	peptide fold	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The spectral properties of the beta B2 mutants , as well as their stabilities against denaturants , resemble those of wild-type beta B2-crystallin , thus indicating that the overall peptide fold of the subunits is not changed significantly .
	manualset3
166218	7	412583	7	NULL	NULL	0	NULL	subunits	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The spectral properties of the beta B2 mutants , as well as their stabilities against denaturants , resemble those of wild-type beta B2-crystallin , thus indicating that the overall peptide fold of the subunits is not changed significantly .
	manualset3
166219	1	412584	7	NULL	NULL	0	NULL	sperm-egg interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The sperm-egg interaction was recorded on videotape or assessed after fixation of the eggs with bound sperm .
	manualset3
166220	2	412584	7	NULL	NULL	0	NULL	videotape	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The sperm-egg interaction was recorded on videotape or assessed after fixation of the eggs with bound sperm .
	manualset3
166221	3	412584	7	NULL	NULL	NULL	NULL	 fixation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The sperm-egg interaction was recorded on videotape or assessed after fixation of the eggs with bound sperm .
	manualset3
166222	5	412584	7	NULL	NULL	NULL	NULL	sperm	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The sperm-egg interaction was recorded on videotape or assessed after fixation of the eggs with bound sperm .
	manualset3
166223	4	412584	7	NULL	NULL	0	NULL	eggs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The sperm-egg interaction was recorded on videotape or assessed after fixation of the eggs with bound sperm .
	manualset3
166224	1	412585	7	NULL	NULL	0	NULL	spheroplasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The spheroplasts of bordetella pertussis .
	manualset3
166225	2	412585	7	NULL	NULL	0	NULL	bordetella pertussis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The spheroplasts of bordetella pertussis .
	manualset3
166226	1	412586	7	NULL	NULL	0	NULL	spin-spin interaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The spin-spin interaction between SQNf and the iron-sulfur cluster N2 was detected as split peaks of the g parallel 2.5 signal with a coupling constant of 1.65 mT , revealing their mutual distance of 8-11 A. The data obtained are consistent with a model in which N2 and two interacting bound ubisemiquinone species are spatially arranged within the hydrophobic domain of Complex I , participating in the vectorial proton translocation .
	manualset3
166227	2	412586	7	NULL	NULL	0	NULL	SQNf	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The spin-spin interaction between SQNf and the iron-sulfur cluster N2 was detected as split peaks of the g parallel 2.5 signal with a coupling constant of 1.65 mT , revealing their mutual distance of 8-11 A. The data obtained are consistent with a model in which N2 and two interacting bound ubisemiquinone species are spatially arranged within the hydrophobic domain of Complex I , participating in the vectorial proton translocation .
	manualset3
166228	3	412586	7	NULL	NULL	0	NULL	iron-sulfur cluster N2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The spin-spin interaction between SQNf and the iron-sulfur cluster N2 was detected as split peaks of the g parallel 2.5 signal with a coupling constant of 1.65 mT , revealing their mutual distance of 8-11 A. The data obtained are consistent with a model in which N2 and two interacting bound ubisemiquinone species are spatially arranged within the hydrophobic domain of Complex I , participating in the vectorial proton translocation .
	manualset3
166229	4	412586	7	NULL	NULL	0	NULL	split peaks 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The spin-spin interaction between SQNf and the iron-sulfur cluster N2 was detected as split peaks of the g parallel 2.5 signal with a coupling constant of 1.65 mT , revealing their mutual distance of 8-11 A. The data obtained are consistent with a model in which N2 and two interacting bound ubisemiquinone species are spatially arranged within the hydrophobic domain of Complex I , participating in the vectorial proton translocation .
	manualset3
166230	5	412586	7	NULL	NULL	0	NULL	g parallel 2.5 signal	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The spin-spin interaction between SQNf and the iron-sulfur cluster N2 was detected as split peaks of the g parallel 2.5 signal with a coupling constant of 1.65 mT , revealing their mutual distance of 8-11 A. The data obtained are consistent with a model in which N2 and two interacting bound ubisemiquinone species are spatially arranged within the hydrophobic domain of Complex I , participating in the vectorial proton translocation .
	manualset3
166231	6	412586	7	NULL	NULL	0	NULL	coupling constant	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The spin-spin interaction between SQNf and the iron-sulfur cluster N2 was detected as split peaks of the g parallel 2.5 signal with a coupling constant of 1.65 mT , revealing their mutual distance of 8-11 A. The data obtained are consistent with a model in which N2 and two interacting bound ubisemiquinone species are spatially arranged within the hydrophobic domain of Complex I , participating in the vectorial proton translocation .
	manualset3
166232	7	412586	7	NULL	NULL	0	NULL	1.65 mT	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The spin-spin interaction between SQNf and the iron-sulfur cluster N2 was detected as split peaks of the g parallel 2.5 signal with a coupling constant of 1.65 mT , revealing their mutual distance of 8-11 A. The data obtained are consistent with a model in which N2 and two interacting bound ubisemiquinone species are spatially arranged within the hydrophobic domain of Complex I , participating in the vectorial proton translocation .
	manualset3
166233	8	412586	7	NULL	NULL	0	NULL	distance	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The spin-spin interaction between SQNf and the iron-sulfur cluster N2 was detected as split peaks of the g parallel 2.5 signal with a coupling constant of 1.65 mT , revealing their mutual distance of 8-11 A. The data obtained are consistent with a model in which N2 and two interacting bound ubisemiquinone species are spatially arranged within the hydrophobic domain of Complex I , participating in the vectorial proton translocation .
	manualset3
166234	9	412586	7	NULL	NULL	0	NULL	8-11 A	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The spin-spin interaction between SQNf and the iron-sulfur cluster N2 was detected as split peaks of the g parallel 2.5 signal with a coupling constant of 1.65 mT , revealing their mutual distance of 8-11 A. The data obtained are consistent with a model in which N2 and two interacting bound ubisemiquinone species are spatially arranged within the hydrophobic domain of Complex I , participating in the vectorial proton translocation .
	manualset3
166235	10	412586	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The spin-spin interaction between SQNf and the iron-sulfur cluster N2 was detected as split peaks of the g parallel 2.5 signal with a coupling constant of 1.65 mT , revealing their mutual distance of 8-11 A. The data obtained are consistent with a model in which N2 and two interacting bound ubisemiquinone species are spatially arranged within the hydrophobic domain of Complex I , participating in the vectorial proton translocation .
	manualset3
166236	11	412586	7	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The spin-spin interaction between SQNf and the iron-sulfur cluster N2 was detected as split peaks of the g parallel 2.5 signal with a coupling constant of 1.65 mT , revealing their mutual distance of 8-11 A. The data obtained are consistent with a model in which N2 and two interacting bound ubisemiquinone species are spatially arranged within the hydrophobic domain of Complex I , participating in the vectorial proton translocation .
	manualset3
166237	12	412586	7	NULL	NULL	NULL	NULL	N2	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The spin-spin interaction between SQNf and the iron-sulfur cluster N2 was detected as split peaks of the g parallel 2.5 signal with a coupling constant of 1.65 mT , revealing their mutual distance of 8-11 A. The data obtained are consistent with a model in which N2 and two interacting bound ubisemiquinone species are spatially arranged within the hydrophobic domain of Complex I , participating in the vectorial proton translocation .
	manualset3
166238	13	412586	7	NULL	NULL	0	NULL	 two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The spin-spin interaction between SQNf and the iron-sulfur cluster N2 was detected as split peaks of the g parallel 2.5 signal with a coupling constant of 1.65 mT , revealing their mutual distance of 8-11 A. The data obtained are consistent with a model in which N2 and two interacting bound ubisemiquinone species are spatially arranged within the hydrophobic domain of Complex I , participating in the vectorial proton translocation .
	manualset3
166239	14	412586	7	NULL	NULL	0	NULL	ubisemiquinone species	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The spin-spin interaction between SQNf and the iron-sulfur cluster N2 was detected as split peaks of the g parallel 2.5 signal with a coupling constant of 1.65 mT , revealing their mutual distance of 8-11 A. The data obtained are consistent with a model in which N2 and two interacting bound ubisemiquinone species are spatially arranged within the hydrophobic domain of Complex I , participating in the vectorial proton translocation .
	manualset3
166240	15	412586	7	NULL	NULL	0	NULL	hydrophobic domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The spin-spin interaction between SQNf and the iron-sulfur cluster N2 was detected as split peaks of the g parallel 2.5 signal with a coupling constant of 1.65 mT , revealing their mutual distance of 8-11 A. The data obtained are consistent with a model in which N2 and two interacting bound ubisemiquinone species are spatially arranged within the hydrophobic domain of Complex I , participating in the vectorial proton translocation .
	manualset3
166241	16	412586	7	NULL	NULL	0	NULL	Complex I	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The spin-spin interaction between SQNf and the iron-sulfur cluster N2 was detected as split peaks of the g parallel 2.5 signal with a coupling constant of 1.65 mT , revealing their mutual distance of 8-11 A. The data obtained are consistent with a model in which N2 and two interacting bound ubisemiquinone species are spatially arranged within the hydrophobic domain of Complex I , participating in the vectorial proton translocation .
	manualset3
166242	17	412586	7	NULL	NULL	0	NULL	vectorial proton translocation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The spin-spin interaction between SQNf and the iron-sulfur cluster N2 was detected as split peaks of the g parallel 2.5 signal with a coupling constant of 1.65 mT , revealing their mutual distance of 8-11 A. The data obtained are consistent with a model in which N2 and two interacting bound ubisemiquinone species are spatially arranged within the hydrophobic domain of Complex I , participating in the vectorial proton translocation .
	manualset3
166243	1	412587	7	NULL	NULL	0	NULL	spin state marker bands	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The spin state marker bands observed from the Mb film in the 1550-1630 cm ( - ) ( 1 ) region ( excitation at 514.5 nm ) are approximately 20 cm ( - ) ( 1 ) higher than those of aqueous metMb having the high spin state .
	manualset3
166244	2	412587	7	NULL	NULL	0	NULL	Mb film	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The spin state marker bands observed from the Mb film in the 1550-1630 cm ( - ) ( 1 ) region ( excitation at 514.5 nm ) are approximately 20 cm ( - ) ( 1 ) higher than those of aqueous metMb having the high spin state .
	manualset3
166245	3	412587	7	NULL	NULL	0	NULL	1550-1630 cm ( - ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The spin state marker bands observed from the Mb film in the 1550-1630 cm ( - ) ( 1 ) region ( excitation at 514.5 nm ) are approximately 20 cm ( - ) ( 1 ) higher than those of aqueous metMb having the high spin state .
	manualset3
166246	4	412587	7	NULL	NULL	0	NULL	region	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The spin state marker bands observed from the Mb film in the 1550-1630 cm ( - ) ( 1 ) region ( excitation at 514.5 nm ) are approximately 20 cm ( - ) ( 1 ) higher than those of aqueous metMb having the high spin state .
	manualset3
166247	5	412587	7	NULL	NULL	0	NULL	excitation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The spin state marker bands observed from the Mb film in the 1550-1630 cm ( - ) ( 1 ) region ( excitation at 514.5 nm ) are approximately 20 cm ( - ) ( 1 ) higher than those of aqueous metMb having the high spin state .
	manualset3
166248	6	412587	7	NULL	NULL	0	NULL	514.5 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The spin state marker bands observed from the Mb film in the 1550-1630 cm ( - ) ( 1 ) region ( excitation at 514.5 nm ) are approximately 20 cm ( - ) ( 1 ) higher than those of aqueous metMb having the high spin state .
	manualset3
166249	7	412587	7	NULL	NULL	0	NULL	20 cm ( - ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The spin state marker bands observed from the Mb film in the 1550-1630 cm ( - ) ( 1 ) region ( excitation at 514.5 nm ) are approximately 20 cm ( - ) ( 1 ) higher than those of aqueous metMb having the high spin state .
	manualset3
166250	8	412587	7	NULL	NULL	0	NULL	aqueous metMb 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The spin state marker bands observed from the Mb film in the 1550-1630 cm ( - ) ( 1 ) region ( excitation at 514.5 nm ) are approximately 20 cm ( - ) ( 1 ) higher than those of aqueous metMb having the high spin state .
	manualset3
166251	9	412587	7	NULL	NULL	0	NULL	high spin state	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The spin state marker bands observed from the Mb film in the 1550-1630 cm ( - ) ( 1 ) region ( excitation at 514.5 nm ) are approximately 20 cm ( - ) ( 1 ) higher than those of aqueous metMb having the high spin state .
	manualset3
166252	1	412588	7	NULL	NULL	0	NULL	splenocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The splenocytes from immunized mice revealed significantly higher natural killer cell activity .
	manualset3
166253	2	412588	7	NULL	NULL	0	NULL	immunized mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The splenocytes from immunized mice revealed significantly higher natural killer cell activity .
	manualset3
166254	3	412588	7	NULL	NULL	0	NULL	natural killer cell activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The splenocytes from immunized mice revealed significantly higher natural killer cell activity .
	manualset3
166255	1	412589	7	NULL	NULL	0	NULL	spoVR gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The spoVR gene was located on the B. subtilis chromosome immediately upstream from , and in the opposite orientation of , the phoAIV gene .
	manualset3
166256	2	412589	7	NULL	NULL	0	NULL	B. subtilis chromosome	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The spoVR gene was located on the B. subtilis chromosome immediately upstream from , and in the opposite orientation of , the phoAIV gene .
	manualset3
166257	3	412589	7	NULL	NULL	0	NULL	 opposite orientation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The spoVR gene was located on the B. subtilis chromosome immediately upstream from , and in the opposite orientation of , the phoAIV gene .
	manualset3
166258	4	412589	7	NULL	NULL	0	NULL	phoAIV gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The spoVR gene was located on the B. subtilis chromosome immediately upstream from , and in the opposite orientation of , the phoAIV gene .
	manualset3
166259	1	412590	7	NULL	NULL	0	NULL	 spread	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The spread of MRSA means that novel targets are required to develop potential inhibitors to combat infections caused by such drug-resistant bacteria .
	manualset3
166260	2	412590	7	NULL	NULL	0	NULL	MRSA	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The spread of MRSA means that novel targets are required to develop potential inhibitors to combat infections caused by such drug-resistant bacteria .
	manualset3
166261	3	412590	7	NULL	NULL	0	NULL	novel targets	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The spread of MRSA means that novel targets are required to develop potential inhibitors to combat infections caused by such drug-resistant bacteria .
	manualset3
166262	4	412590	7	NULL	NULL	0	NULL	potential inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The spread of MRSA means that novel targets are required to develop potential inhibitors to combat infections caused by such drug-resistant bacteria .
	manualset3
166263	5	412590	7	NULL	NULL	0	NULL	infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The spread of MRSA means that novel targets are required to develop potential inhibitors to combat infections caused by such drug-resistant bacteria .
	manualset3
166264	6	412590	7	NULL	NULL	0	NULL	drug-resistant bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The spread of MRSA means that novel targets are required to develop potential inhibitors to combat infections caused by such drug-resistant bacteria .
	manualset3
166265	1	412591	7	NULL	NULL	0	NULL	new class	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , we developed a new class of NNRTIs , the 1 , 4-dihydro-2H-3 , 1-benzoxazin-2-ones .
	manualset3
166266	2	412591	7	NULL	NULL	0	NULL	NNRTIs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , we developed a new class of NNRTIs , the 1 , 4-dihydro-2H-3 , 1-benzoxazin-2-ones .
	manualset3
166267	3	412591	7	NULL	NULL	0	NULL	1 , 4-dihydro-2H-3 , 1-benzoxazin-2-ones	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , we developed a new class of NNRTIs , the 1 , 4-dihydro-2H-3 , 1-benzoxazin-2-ones .
	manualset3
166268	1	412592	7	NULL	NULL	0	NULL	 stability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The stability of bromelain : Fab complex ( 1 : 1 stoichiometry ) was investigated by far and near-UV CD and fluorescence measurements .
	manualset3
166269	2	412592	7	NULL	NULL	0	NULL	bromelain : Fab complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The stability of bromelain : Fab complex ( 1 : 1 stoichiometry ) was investigated by far and near-UV CD and fluorescence measurements .
	manualset3
166270	3	412592	7	NULL	NULL	NULL	NULL	1 : 1 stoichiometry	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The stability of bromelain : Fab complex ( 1 : 1 stoichiometry ) was investigated by far and near-UV CD and fluorescence measurements .
	manualset3
166271	4	412592	7	NULL	NULL	0	NULL	far and near-UV CD and fluorescence measurements	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The stability of bromelain : Fab complex ( 1 : 1 stoichiometry ) was investigated by far and near-UV CD and fluorescence measurements .
	manualset3
166272	1	412593	7	NULL	NULL	0	NULL	stability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The stability of oseltamivir in oral aqueous solutions containing the preservative sodium benzoate was studied by a stability indicating HPLC-method .
	manualset3
166273	2	412593	7	NULL	NULL	0	NULL	oseltamivir	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The stability of oseltamivir in oral aqueous solutions containing the preservative sodium benzoate was studied by a stability indicating HPLC-method .
	manualset3
166274	3	412593	7	NULL	NULL	0	NULL	oral aqueous solutions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The stability of oseltamivir in oral aqueous solutions containing the preservative sodium benzoate was studied by a stability indicating HPLC-method .
	manualset3
166275	4	412593	7	NULL	NULL	0	NULL	preservative sodium benzoate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The stability of oseltamivir in oral aqueous solutions containing the preservative sodium benzoate was studied by a stability indicating HPLC-method .
	manualset3
166276	5	412593	7	NULL	NULL	0	NULL	 stability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The stability of oseltamivir in oral aqueous solutions containing the preservative sodium benzoate was studied by a stability indicating HPLC-method .
	manualset3
166277	6	412593	7	NULL	NULL	0	NULL	 HPLC-method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The stability of oseltamivir in oral aqueous solutions containing the preservative sodium benzoate was studied by a stability indicating HPLC-method .
	manualset3
166278	1	412594	7	NULL	NULL	0	NULL	 stability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The stability of vitamin A acetate in aqueous cetomacrogol solutions : a spectroscopic study .
	manualset3
166279	2	412594	7	NULL	NULL	0	NULL	vitamin A acetate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The stability of vitamin A acetate in aqueous cetomacrogol solutions : a spectroscopic study .
	manualset3
166280	3	412594	7	NULL	NULL	0	NULL	aqueous cetomacrogol solutions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The stability of vitamin A acetate in aqueous cetomacrogol solutions : a spectroscopic study .
	manualset3
166281	4	412594	7	NULL	NULL	0	NULL	spectroscopic study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The stability of vitamin A acetate in aqueous cetomacrogol solutions : a spectroscopic study .
	manualset3
166282	1	412595	7	NULL	NULL	0	NULL	stable patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The stable patient with an occult cardiac injury can represent a diagnostic dilemma .
	manualset3
166283	2	412595	7	NULL	NULL	0	NULL	occult cardiac injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The stable patient with an occult cardiac injury can represent a diagnostic dilemma .
	manualset3
166284	3	412595	7	NULL	NULL	0	NULL	diagnostic dilemma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The stable patient with an occult cardiac injury can represent a diagnostic dilemma .
	manualset3
166285	1	412596	7	NULL	NULL	0	NULL	staining	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The staining for AR showed only minor cyclic changes .
	manualset3
166286	2	412596	7	NULL	NULL	0	NULL	AR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The staining for AR showed only minor cyclic changes .
	manualset3
166287	3	412596	7	NULL	NULL	0	NULL	minor cyclic changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The staining for AR showed only minor cyclic changes .
	manualset3
166288	1	412597	7	NULL	NULL	0	NULL	stakeholders	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The stakeholders agreed that they must be involved in the role development process , i.e. , implementation must not be a top-down initiative .
	manualset3
166289	2	412597	7	NULL	NULL	0	NULL	 role development process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The stakeholders agreed that they must be involved in the role development process , i.e. , implementation must not be a top-down initiative .
	manualset3
166290	3	412597	7	NULL	NULL	0	NULL	implementation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The stakeholders agreed that they must be involved in the role development process , i.e. , implementation must not be a top-down initiative .
	manualset3
166291	4	412597	7	NULL	NULL	0	NULL	top-down initiative	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The stakeholders agreed that they must be involved in the role development process , i.e. , implementation must not be a top-down initiative .
	manualset3
166292	1	412598	7	NULL	NULL	0	NULL	standard lipid profile	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The standard lipid profile has an enormous scientific evidence base and has provided simple clinical lipid-altering goals focused on low-density lipoprotein ( LDL ) cholesterol that have been shown to reduce coronary heart disease .
	manualset3
166293	2	412598	7	NULL	NULL	NULL	NULL	scientific evidence base	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The standard lipid profile has an enormous scientific evidence base and has provided simple clinical lipid-altering goals focused on low-density lipoprotein ( LDL ) cholesterol that have been shown to reduce coronary heart disease .
	manualset3
166294	3	412598	7	NULL	NULL	NULL	NULL	simple clinical lipid-altering goals	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The standard lipid profile has an enormous scientific evidence base and has provided simple clinical lipid-altering goals focused on low-density lipoprotein ( LDL ) cholesterol that have been shown to reduce coronary heart disease .
	manualset3
166295	4	412598	7	NULL	NULL	0	NULL	 low-density lipoprotein ( LDL ) cholesterol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The standard lipid profile has an enormous scientific evidence base and has provided simple clinical lipid-altering goals focused on low-density lipoprotein ( LDL ) cholesterol that have been shown to reduce coronary heart disease .
	manualset3
166296	5	412598	7	NULL	NULL	0	NULL	coronary heart disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The standard lipid profile has an enormous scientific evidence base and has provided simple clinical lipid-altering goals focused on low-density lipoprotein ( LDL ) cholesterol that have been shown to reduce coronary heart disease .
	manualset3
166297	1	412599	7	NULL	NULL	NULL	NULL	standard method 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The standard method used to detect and monitor ketonemia in human medicine is measurement of serum or whole blood beta-hydroxybutyrate ( HOB ) .
	manualset3
166298	2	412599	7	NULL	NULL	0	NULL	ketonemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The standard method used to detect and monitor ketonemia in human medicine is measurement of serum or whole blood beta-hydroxybutyrate ( HOB ) .
	manualset3
166299	3	412599	7	NULL	NULL	0	NULL	human medicine	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The standard method used to detect and monitor ketonemia in human medicine is measurement of serum or whole blood beta-hydroxybutyrate ( HOB ) .
	manualset3
166300	4	412599	7	NULL	NULL	0	NULL	measurement	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The standard method used to detect and monitor ketonemia in human medicine is measurement of serum or whole blood beta-hydroxybutyrate ( HOB ) .
	manualset3
166301	5	412599	7	NULL	NULL	0	NULL	serum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The standard method used to detect and monitor ketonemia in human medicine is measurement of serum or whole blood beta-hydroxybutyrate ( HOB ) .
	manualset3
166302	6	412599	7	NULL	NULL	0	NULL	whole blood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The standard method used to detect and monitor ketonemia in human medicine is measurement of serum or whole blood beta-hydroxybutyrate ( HOB ) .
	manualset3
166303	7	412599	7	NULL	NULL	0	NULL	beta-hydroxybutyrate ( HOB )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The standard method used to detect and monitor ketonemia in human medicine is measurement of serum or whole blood beta-hydroxybutyrate ( HOB ) .
	manualset3
166304	1	412600	7	NULL	NULL	0	NULL	starvation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The starvation and dehydration may then be the important factors for death that follows oral dosing with organolead and organotin compounds .
	manualset3
166305	2	412600	7	NULL	NULL	0	NULL	dehydration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The starvation and dehydration may then be the important factors for death that follows oral dosing with organolead and organotin compounds .
	manualset3
166306	3	412600	7	NULL	NULL	0	NULL	 important factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The starvation and dehydration may then be the important factors for death that follows oral dosing with organolead and organotin compounds .
	manualset3
166307	4	412600	7	NULL	NULL	0	NULL	death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The starvation and dehydration may then be the important factors for death that follows oral dosing with organolead and organotin compounds .
	manualset3
166308	5	412600	7	NULL	NULL	0	NULL	oral dosing	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The starvation and dehydration may then be the important factors for death that follows oral dosing with organolead and organotin compounds .
	manualset3
166309	6	412600	7	NULL	NULL	0	NULL	organolead compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The starvation and dehydration may then be the important factors for death that follows oral dosing with organolead and organotin compounds .
	manualset3
166310	7	412600	7	NULL	NULL	0	NULL	organotin compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The starvation and dehydration may then be the important factors for death that follows oral dosing with organolead and organotin compounds .
	manualset3
166311	1	412601	7	NULL	NULL	NULL	NULL	 static vestibule resistance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The static vestibule resistance in the total nasal resistance was obtained by calculating the difference between nasal flows with and without the dilator .
	manualset3
166312	2	412601	7	NULL	NULL	NULL	NULL	total nasal resistance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The static vestibule resistance in the total nasal resistance was obtained by calculating the difference between nasal flows with and without the dilator .
	manualset3
166313	3	412601	7	NULL	NULL	0	NULL	 difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The static vestibule resistance in the total nasal resistance was obtained by calculating the difference between nasal flows with and without the dilator .
	manualset3
166314	4	412601	7	NULL	NULL	0	NULL	nasal flows	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The static vestibule resistance in the total nasal resistance was obtained by calculating the difference between nasal flows with and without the dilator .
	manualset3
166315	5	412601	7	NULL	NULL	0	NULL	dilator	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The static vestibule resistance in the total nasal resistance was obtained by calculating the difference between nasal flows with and without the dilator .
	manualset3
166316	1	412602	7	NULL	NULL	NULL	NULL	stationary state	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The stationary state is determined by the balance between the heating of the dot electrons by the perturbation and cooling by electron exchange with the cold contacts .
	manualset3
166317	2	412602	7	NULL	NULL	NULL	NULL	balance	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The stationary state is determined by the balance between the heating of the dot electrons by the perturbation and cooling by electron exchange with the cold contacts .
	manualset3
166318	3	412602	7	NULL	NULL	NULL	NULL	heating	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The stationary state is determined by the balance between the heating of the dot electrons by the perturbation and cooling by electron exchange with the cold contacts .
	manualset3
166319	4	412602	7	NULL	NULL	0	NULL	 dot electrons 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The stationary state is determined by the balance between the heating of the dot electrons by the perturbation and cooling by electron exchange with the cold contacts .
	manualset3
166320	5	412602	7	NULL	NULL	NULL	NULL	perturbation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The stationary state is determined by the balance between the heating of the dot electrons by the perturbation and cooling by electron exchange with the cold contacts .
	manualset3
166321	6	412602	7	NULL	NULL	NULL	NULL	 cooling 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The stationary state is determined by the balance between the heating of the dot electrons by the perturbation and cooling by electron exchange with the cold contacts .
	manualset3
166322	7	412602	7	NULL	NULL	0	NULL	electron exchange	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The stationary state is determined by the balance between the heating of the dot electrons by the perturbation and cooling by electron exchange with the cold contacts .
	manualset3
166323	8	412602	7	NULL	NULL	0	NULL	cold contacts	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The stationary state is determined by the balance between the heating of the dot electrons by the perturbation and cooling by electron exchange with the cold contacts .
	manualset3
166324	1	412603	7	NULL	NULL	0	NULL	statistical associations 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The statistical associations between stress and cardiovascular and other prevalent diseases have not been explained .
	manualset3
166325	2	412603	7	NULL	NULL	0	NULL	 stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The statistical associations between stress and cardiovascular and other prevalent diseases have not been explained .
	manualset3
166326	3	412603	7	NULL	NULL	0	NULL	cardiovascular diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The statistical associations between stress and cardiovascular and other prevalent diseases have not been explained .
	manualset3
173647	4	412603	7	NULL	NULL	0	NULL	prevalent diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The statistical associations between stress and cardiovascular and other prevalent diseases have not been explained .
	manualset3
166327	1	412604	7	NULL	NULL	0	NULL	statistical indices	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The statistical indices such as mean square error ( MSE ) , maximum absolute error ( MAE ) and peak signal-to-noise ratio ( PSNR ) were used to quantify the effect of wavelet compression of selected images .
	manualset3
166328	2	412604	7	NULL	NULL	NULL	NULL	mean square error ( MSE )	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The statistical indices such as mean square error ( MSE ) , maximum absolute error ( MAE ) and peak signal-to-noise ratio ( PSNR ) were used to quantify the effect of wavelet compression of selected images .
	manualset3
166329	3	412604	7	NULL	NULL	NULL	NULL	maximum absolute error ( MAE )	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The statistical indices such as mean square error ( MSE ) , maximum absolute error ( MAE ) and peak signal-to-noise ratio ( PSNR ) were used to quantify the effect of wavelet compression of selected images .
	manualset3
166330	4	412604	7	NULL	NULL	NULL	NULL	peak signal-to-noise ratio ( PSNR )	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The statistical indices such as mean square error ( MSE ) , maximum absolute error ( MAE ) and peak signal-to-noise ratio ( PSNR ) were used to quantify the effect of wavelet compression of selected images .
	manualset3
166331	5	412604	7	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The statistical indices such as mean square error ( MSE ) , maximum absolute error ( MAE ) and peak signal-to-noise ratio ( PSNR ) were used to quantify the effect of wavelet compression of selected images .
	manualset3
166332	6	412604	7	NULL	NULL	0	NULL	wavelet compression 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The statistical indices such as mean square error ( MSE ) , maximum absolute error ( MAE ) and peak signal-to-noise ratio ( PSNR ) were used to quantify the effect of wavelet compression of selected images .
	manualset3
166333	7	412604	7	NULL	NULL	0	NULL	 images	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The statistical indices such as mean square error ( MSE ) , maximum absolute error ( MAE ) and peak signal-to-noise ratio ( PSNR ) were used to quantify the effect of wavelet compression of selected images .
	manualset3
166334	1	412605	7	NULL	NULL	0	NULL	statistical method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The statistical method consisted of an ANOVA after log-transformation of the working times .
	manualset3
166335	2	412605	7	NULL	NULL	0	NULL	ANOVA	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The statistical method consisted of an ANOVA after log-transformation of the working times .
	manualset3
166336	3	412605	7	NULL	NULL	0	NULL	 log-transformation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The statistical method consisted of an ANOVA after log-transformation of the working times .
	manualset3
166337	4	412605	7	NULL	NULL	0	NULL	working times	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The statistical method consisted of an ANOVA after log-transformation of the working times .
	manualset3
166338	1	412606	7	NULL	NULL	0	NULL	small differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The statistically significant but only very small differences in the pharmacokinetic parameters and in the urinary excretion were observed over the wide range of dose ( 0.20 , 2.0 and 20 mg/kg ) .
	manualset3
166339	2	412606	7	NULL	NULL	0	NULL	pharmacokinetic parameters	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The statistically significant but only very small differences in the pharmacokinetic parameters and in the urinary excretion were observed over the wide range of dose ( 0.20 , 2.0 and 20 mg/kg ) .
	manualset3
166340	3	412606	7	NULL	NULL	0	NULL	urinary excretion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The statistically significant but only very small differences in the pharmacokinetic parameters and in the urinary excretion were observed over the wide range of dose ( 0.20 , 2.0 and 20 mg/kg ) .
	manualset3
166341	4	412606	7	NULL	NULL	0	NULL	wide range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The statistically significant but only very small differences in the pharmacokinetic parameters and in the urinary excretion were observed over the wide range of dose ( 0.20 , 2.0 and 20 mg/kg ) .
	manualset3
166342	5	412606	7	NULL	NULL	0	NULL	 dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The statistically significant but only very small differences in the pharmacokinetic parameters and in the urinary excretion were observed over the wide range of dose ( 0.20 , 2.0 and 20 mg/kg ) .
	manualset3
166343	6	412606	7	NULL	NULL	0	NULL	 0.20 , 2.0 and 20 mg/kg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The statistically significant but only very small differences in the pharmacokinetic parameters and in the urinary excretion were observed over the wide range of dose ( 0.20 , 2.0 and 20 mg/kg ) .
	manualset3
166344	1	412607	7	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The statistically significant difference of immunoreactivity for p-STAT3 between the CRA and adenoma , and between the CRA and normal mucosae was identified .
	manualset3
166345	2	412607	7	NULL	NULL	0	NULL	immunoreactivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The statistically significant difference of immunoreactivity for p-STAT3 between the CRA and adenoma , and between the CRA and normal mucosae was identified .
	manualset3
166346	3	412607	7	NULL	NULL	0	NULL	p-STAT3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The statistically significant difference of immunoreactivity for p-STAT3 between the CRA and adenoma , and between the CRA and normal mucosae was identified .
	manualset3
166347	4	412607	7	NULL	NULL	0	NULL	CRA	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The statistically significant difference of immunoreactivity for p-STAT3 between the CRA and adenoma , and between the CRA and normal mucosae was identified .
	manualset3
166348	5	412607	7	NULL	NULL	0	NULL	adenoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The statistically significant difference of immunoreactivity for p-STAT3 between the CRA and adenoma , and between the CRA and normal mucosae was identified .
	manualset3
166349	6	412607	7	NULL	NULL	0	NULL	CRA	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The statistically significant difference of immunoreactivity for p-STAT3 between the CRA and adenoma , and between the CRA and normal mucosae was identified .
	manualset3
166350	7	412607	7	NULL	NULL	0	NULL	 normal mucosae	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The statistically significant difference of immunoreactivity for p-STAT3 between the CRA and adenoma , and between the CRA and normal mucosae was identified .
	manualset3
166351	1	412608	7	NULL	NULL	0	NULL	status	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The status of drinking in Japan ) .
	manualset3
166352	2	412608	7	NULL	NULL	0	NULL	drinking 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The status of drinking in Japan ) .
	manualset3
166353	3	412608	7	NULL	NULL	0	NULL	Japan 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The status of drinking in Japan ) .
	manualset3
166354	1	412609	7	NULL	NULL	0	NULL	status	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The status of phospholamban ( PLB ) phosphorylation in the ischemia-reperfused hearts remains controversial .
	manualset3
166355	2	412609	7	NULL	NULL	NULL	NULL	phospholamban ( PLB ) phosphorylation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The status of phospholamban ( PLB ) phosphorylation in the ischemia-reperfused hearts remains controversial .
	manualset3
166356	3	412609	7	NULL	NULL	0	NULL	ischemia-reperfused hearts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The status of phospholamban ( PLB ) phosphorylation in the ischemia-reperfused hearts remains controversial .
	manualset3
166357	1	412610	7	NULL	NULL	0	NULL	steady-state mRNA levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The steady-state mRNA levels of the proliferating cell nuclear antigen ( PCNA ) gene are growth regulated .
	manualset3
166358	2	412610	7	NULL	NULL	0	NULL	proliferating cell nuclear antigen ( PCNA ) gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The steady-state mRNA levels of the proliferating cell nuclear antigen ( PCNA ) gene are growth regulated .
	manualset3
166359	1	412611	7	NULL	NULL	0	NULL	steady state intestinal extraction ratios 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The steady state intestinal extraction ratios ( E1 , 0.33 to 0.06 ) and hepatic extraction ratios ( EH , 0.84 to 0.37 ) were highly concentration dependent , decreasing with increasing GAM concentrations .
	manualset3
166360	2	412611	7	NULL	NULL	0	NULL	E1 , 0.33 to 0.06	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The steady state intestinal extraction ratios ( E1 , 0.33 to 0.06 ) and hepatic extraction ratios ( EH , 0.84 to 0.37 ) were highly concentration dependent , decreasing with increasing GAM concentrations .
	manualset3
166361	3	412611	7	NULL	NULL	0	NULL	hepatic extraction ratios	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The steady state intestinal extraction ratios ( E1 , 0.33 to 0.06 ) and hepatic extraction ratios ( EH , 0.84 to 0.37 ) were highly concentration dependent , decreasing with increasing GAM concentrations .
	manualset3
166362	4	412611	7	NULL	NULL	0	NULL	EH , 0.84 to 0.37 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The steady state intestinal extraction ratios ( E1 , 0.33 to 0.06 ) and hepatic extraction ratios ( EH , 0.84 to 0.37 ) were highly concentration dependent , decreasing with increasing GAM concentrations .
	manualset3
166363	5	412611	7	NULL	NULL	NULL	NULL	GAM concentrations	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The steady state intestinal extraction ratios ( E1 , 0.33 to 0.06 ) and hepatic extraction ratios ( EH , 0.84 to 0.37 ) were highly concentration dependent , decreasing with increasing GAM concentrations .
	manualset3
166365	1	412612	7	NULL	NULL	0	NULL	stenoses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The stenoses were quite discrete ( 4 + / - 5 mm ) and calcified in the majority ( 40 ) of the 53 patients .
	manualset3
166366	2	412612	7	NULL	NULL	0	NULL	 4 + / - 5 mm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The stenoses were quite discrete ( 4 + / - 5 mm ) and calcified in the majority ( 40 ) of the 53 patients .
	manualset3
166367	4	412612	7	NULL	NULL	NULL	NULL	majority ( 40 )	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The stenoses were quite discrete ( 4 + / - 5 mm ) and calcified in the majority ( 40 ) of the 53 patients .
	manualset3
166368	5	412612	7	NULL	NULL	NULL	NULL	53 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The stenoses were quite discrete ( 4 + / - 5 mm ) and calcified in the majority ( 40 ) of the 53 patients .
	manualset3
167233	3	412612	7	NULL	NULL	NULL	NULL	 calcified	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The stenoses were quite discrete ( 4 + / - 5 mm ) and calcified in the majority ( 40 ) of the 53 patients .
	manualset3
166369	1	412613	7	NULL	NULL	0	NULL	 steps	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The steps in designing a controlled trial to evaluate a new treatment for inoperable carcinoma of the bronchus are described .
	manualset3
166370	2	412613	7	NULL	NULL	0	NULL	controlled trial	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The steps in designing a controlled trial to evaluate a new treatment for inoperable carcinoma of the bronchus are described .
	manualset3
166371	3	412613	7	NULL	NULL	0	NULL	new treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The steps in designing a controlled trial to evaluate a new treatment for inoperable carcinoma of the bronchus are described .
	manualset3
166372	4	412613	7	NULL	NULL	0	NULL	inoperable carcinoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The steps in designing a controlled trial to evaluate a new treatment for inoperable carcinoma of the bronchus are described .
	manualset3
166373	5	412613	7	NULL	NULL	0	NULL	bronchus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The steps in designing a controlled trial to evaluate a new treatment for inoperable carcinoma of the bronchus are described .
	manualset3
166374	1	412614	7	NULL	NULL	0	NULL	stimulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulation of 45Ca ( 2 + ) - uptake by K ( + ) - depolarization , unlike that induced by glucose , was not sensitive to norepinephrine , starvation or fatty acid oxidation inhibitors .
	manualset3
166375	2	412614	7	NULL	NULL	0	NULL	45Ca ( 2 + ) - uptake	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulation of 45Ca ( 2 + ) - uptake by K ( + ) - depolarization , unlike that induced by glucose , was not sensitive to norepinephrine , starvation or fatty acid oxidation inhibitors .
	manualset3
166376	3	412614	7	NULL	NULL	0	NULL	K ( + ) - depolarization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulation of 45Ca ( 2 + ) - uptake by K ( + ) - depolarization , unlike that induced by glucose , was not sensitive to norepinephrine , starvation or fatty acid oxidation inhibitors .
	manualset3
166377	4	412614	7	NULL	NULL	0	NULL	glucose	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulation of 45Ca ( 2 + ) - uptake by K ( + ) - depolarization , unlike that induced by glucose , was not sensitive to norepinephrine , starvation or fatty acid oxidation inhibitors .
	manualset3
166378	5	412614	7	NULL	NULL	0	NULL	 norepinephrine	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulation of 45Ca ( 2 + ) - uptake by K ( + ) - depolarization , unlike that induced by glucose , was not sensitive to norepinephrine , starvation or fatty acid oxidation inhibitors .
	manualset3
166379	6	412614	7	NULL	NULL	0	NULL	starvation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulation of 45Ca ( 2 + ) - uptake by K ( + ) - depolarization , unlike that induced by glucose , was not sensitive to norepinephrine , starvation or fatty acid oxidation inhibitors .
	manualset3
166380	7	412614	7	NULL	NULL	0	NULL	fatty acid oxidation inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulation of 45Ca ( 2 + ) - uptake by K ( + ) - depolarization , unlike that induced by glucose , was not sensitive to norepinephrine , starvation or fatty acid oxidation inhibitors .
	manualset3
166381	1	412615	7	NULL	NULL	0	NULL	 stimulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulation of PKC activity by VEGF was preceded by the activation of phospholipase Cgamma ( PLCgamma ) .
	manualset3
166382	2	412615	7	NULL	NULL	0	NULL	PKC activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulation of PKC activity by VEGF was preceded by the activation of phospholipase Cgamma ( PLCgamma ) .
	manualset3
166383	3	412615	7	NULL	NULL	0	NULL	VEGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulation of PKC activity by VEGF was preceded by the activation of phospholipase Cgamma ( PLCgamma ) .
	manualset3
166384	4	412615	7	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulation of PKC activity by VEGF was preceded by the activation of phospholipase Cgamma ( PLCgamma ) .
	manualset3
166385	5	412615	7	NULL	NULL	0	NULL	phospholipase Cgamma ( PLCgamma )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulation of PKC activity by VEGF was preceded by the activation of phospholipase Cgamma ( PLCgamma ) .
	manualset3
166386	1	412616	7	NULL	NULL	0	NULL	evidence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Accumulating evidence implicates oxidatively modified low density lipoproteins ( LDL ) in vascular dysfunction in atherosclerosis and oxidized LDL have been localized with in atherosclerotic lesions .
	manualset3
166387	2	412616	7	NULL	NULL	0	NULL	oxidatively modified low density lipoproteins ( LDL )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Accumulating evidence implicates oxidatively modified low density lipoproteins ( LDL ) in vascular dysfunction in atherosclerosis and oxidized LDL have been localized with in atherosclerotic lesions .
	manualset3
166388	3	412616	7	NULL	NULL	0	NULL	vascular dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Accumulating evidence implicates oxidatively modified low density lipoproteins ( LDL ) in vascular dysfunction in atherosclerosis and oxidized LDL have been localized with in atherosclerotic lesions .
	manualset3
166389	4	412616	7	NULL	NULL	0	NULL	atherosclerosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Accumulating evidence implicates oxidatively modified low density lipoproteins ( LDL ) in vascular dysfunction in atherosclerosis and oxidized LDL have been localized with in atherosclerotic lesions .
	manualset3
166390	5	412616	7	NULL	NULL	0	NULL	oxidized LDL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Accumulating evidence implicates oxidatively modified low density lipoproteins ( LDL ) in vascular dysfunction in atherosclerosis and oxidized LDL have been localized with in atherosclerotic lesions .
	manualset3
166391	6	412616	7	NULL	NULL	0	NULL	atherosclerotic lesions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Accumulating evidence implicates oxidatively modified low density lipoproteins ( LDL ) in vascular dysfunction in atherosclerosis and oxidized LDL have been localized with in atherosclerotic lesions .
	manualset3
166392	1	412617	7	NULL	NULL	0	NULL	stimulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulation of glycogen synthesis and of glycogen synthetase in the liver by the administration of glucose .
	manualset3
166393	2	412617	7	NULL	NULL	0	NULL	glycogen synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulation of glycogen synthesis and of glycogen synthetase in the liver by the administration of glucose .
	manualset3
166394	3	412617	7	NULL	NULL	0	NULL	 glycogen synthetase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulation of glycogen synthesis and of glycogen synthetase in the liver by the administration of glucose .
	manualset3
166395	4	412617	7	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulation of glycogen synthesis and of glycogen synthetase in the liver by the administration of glucose .
	manualset3
166396	5	412617	7	NULL	NULL	0	NULL	administration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulation of glycogen synthesis and of glycogen synthetase in the liver by the administration of glucose .
	manualset3
166397	6	412617	7	NULL	NULL	0	NULL	glucose	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulation of glycogen synthesis and of glycogen synthetase in the liver by the administration of glucose .
	manualset3
166398	1	412618	7	NULL	NULL	0	NULL	 stimulative effect 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulative effect of P-450scc on 11 beta-hydroxylase activity diminished by the addition of protein-free liposomes to proteoliposomes containing P-45011 beta and P-450scc , thus showing P-450scc to interact with P-45011 beta in the same membranes .
	manualset3
166399	2	412618	7	NULL	NULL	0	NULL	P-450scc	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulative effect of P-450scc on 11 beta-hydroxylase activity diminished by the addition of protein-free liposomes to proteoliposomes containing P-45011 beta and P-450scc , thus showing P-450scc to interact with P-45011 beta in the same membranes .
	manualset3
166400	3	412618	7	NULL	NULL	0	NULL	11 beta-hydroxylase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulative effect of P-450scc on 11 beta-hydroxylase activity diminished by the addition of protein-free liposomes to proteoliposomes containing P-45011 beta and P-450scc , thus showing P-450scc to interact with P-45011 beta in the same membranes .
	manualset3
166401	4	412618	7	NULL	NULL	NULL	NULL	protein-free liposomes	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The stimulative effect of P-450scc on 11 beta-hydroxylase activity diminished by the addition of protein-free liposomes to proteoliposomes containing P-45011 beta and P-450scc , thus showing P-450scc to interact with P-45011 beta in the same membranes .
	manualset3
166402	5	412618	7	NULL	NULL	0	NULL	proteoliposomes 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulative effect of P-450scc on 11 beta-hydroxylase activity diminished by the addition of protein-free liposomes to proteoliposomes containing P-45011 beta and P-450scc , thus showing P-450scc to interact with P-45011 beta in the same membranes .
	manualset3
166403	6	412618	7	NULL	NULL	0	NULL	P-45011 beta	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulative effect of P-450scc on 11 beta-hydroxylase activity diminished by the addition of protein-free liposomes to proteoliposomes containing P-45011 beta and P-450scc , thus showing P-450scc to interact with P-45011 beta in the same membranes .
	manualset3
166404	7	412618	7	NULL	NULL	0	NULL	P-450scc	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulative effect of P-450scc on 11 beta-hydroxylase activity diminished by the addition of protein-free liposomes to proteoliposomes containing P-45011 beta and P-450scc , thus showing P-450scc to interact with P-45011 beta in the same membranes .
	manualset3
166405	8	412618	7	NULL	NULL	0	NULL	P-450scc	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulative effect of P-450scc on 11 beta-hydroxylase activity diminished by the addition of protein-free liposomes to proteoliposomes containing P-45011 beta and P-450scc , thus showing P-450scc to interact with P-45011 beta in the same membranes .
	manualset3
166406	9	412618	7	NULL	NULL	0	NULL	P-45011 beta	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulative effect of P-450scc on 11 beta-hydroxylase activity diminished by the addition of protein-free liposomes to proteoliposomes containing P-45011 beta and P-450scc , thus showing P-450scc to interact with P-45011 beta in the same membranes .
	manualset3
166407	10	412618	7	NULL	NULL	0	NULL	membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulative effect of P-450scc on 11 beta-hydroxylase activity diminished by the addition of protein-free liposomes to proteoliposomes containing P-45011 beta and P-450scc , thus showing P-450scc to interact with P-45011 beta in the same membranes .
	manualset3
166408	1	412619	7	NULL	NULL	0	NULL	stimulatory action 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulatory action of heparan sulfate was mediated , at least in part , by increased production of IL-1 , because the increased splenocyte proliferation induced by heparan sulfate was substantially inhibited by anti-murine IL-1 alpha-antibodies .
	manualset3
166409	2	412619	7	NULL	NULL	0	NULL	heparan sulfate	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulatory action of heparan sulfate was mediated , at least in part , by increased production of IL-1 , because the increased splenocyte proliferation induced by heparan sulfate was substantially inhibited by anti-murine IL-1 alpha-antibodies .
	manualset3
166410	3	412619	7	NULL	NULL	NULL	NULL	increased production 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The stimulatory action of heparan sulfate was mediated , at least in part , by increased production of IL-1 , because the increased splenocyte proliferation induced by heparan sulfate was substantially inhibited by anti-murine IL-1 alpha-antibodies .
	manualset3
166411	4	412619	7	NULL	NULL	0	NULL	increased splenocyte proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulatory action of heparan sulfate was mediated , at least in part , by increased production of IL-1 , because the increased splenocyte proliferation induced by heparan sulfate was substantially inhibited by anti-murine IL-1 alpha-antibodies .
	manualset3
166412	5	412619	7	NULL	NULL	0	NULL	heparan sulfate 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulatory action of heparan sulfate was mediated , at least in part , by increased production of IL-1 , because the increased splenocyte proliferation induced by heparan sulfate was substantially inhibited by anti-murine IL-1 alpha-antibodies .
	manualset3
166413	6	412619	7	NULL	NULL	0	NULL	anti-murine IL-1 alpha-antibodies	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulatory action of heparan sulfate was mediated , at least in part , by increased production of IL-1 , because the increased splenocyte proliferation induced by heparan sulfate was substantially inhibited by anti-murine IL-1 alpha-antibodies .
	manualset3
166414	7	412619	7	NULL	NULL	0	NULL	 IL-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulatory action of heparan sulfate was mediated , at least in part , by increased production of IL-1 , because the increased splenocyte proliferation induced by heparan sulfate was substantially inhibited by anti-murine IL-1 alpha-antibodies .
	manualset3
166415	1	412620	7	NULL	NULL	0	NULL	stimulatory effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulatory effect was inhibited by propranolol , but not by atenolol or phentolamine , in a concentration-dependent manner and was mimicked by salbutamol .
	manualset3
166416	2	412620	7	NULL	NULL	0	NULL	propranolol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulatory effect was inhibited by propranolol , but not by atenolol or phentolamine , in a concentration-dependent manner and was mimicked by salbutamol .
	manualset3
166417	3	412620	7	NULL	NULL	0	NULL	atenolol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulatory effect was inhibited by propranolol , but not by atenolol or phentolamine , in a concentration-dependent manner and was mimicked by salbutamol .
	manualset3
166418	4	412620	7	NULL	NULL	0	NULL	phentolamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulatory effect was inhibited by propranolol , but not by atenolol or phentolamine , in a concentration-dependent manner and was mimicked by salbutamol .
	manualset3
166419	5	412620	7	NULL	NULL	0	NULL	 concentration-dependent manner	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulatory effect was inhibited by propranolol , but not by atenolol or phentolamine , in a concentration-dependent manner and was mimicked by salbutamol .
	manualset3
166420	6	412620	7	NULL	NULL	0	NULL	salbutamol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The stimulatory effect was inhibited by propranolol , but not by atenolol or phentolamine , in a concentration-dependent manner and was mimicked by salbutamol .
	manualset3
166421	1	412621	7	NULL	NULL	0	NULL	 stones	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The stones in 19 of the 23 patients in the multiple stone group remained stable throughout the study , while stones in 4 grew .
	manualset3
166422	2	412621	7	NULL	NULL	NULL	NULL	19 of the 23 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The stones in 19 of the 23 patients in the multiple stone group remained stable throughout the study , while stones in 4 grew .
	manualset3
166424	4	412621	7	NULL	NULL	0	NULL	multiple stone group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The stones in 19 of the 23 patients in the multiple stone group remained stable throughout the study , while stones in 4 grew .
	manualset3
166426	6	412621	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The stones in 19 of the 23 patients in the multiple stone group remained stable throughout the study , while stones in 4 grew .
	manualset3
166427	7	412621	7	NULL	NULL	0	NULL	stones	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The stones in 19 of the 23 patients in the multiple stone group remained stable throughout the study , while stones in 4 grew .
	manualset3
166428	8	412621	7	NULL	NULL	NULL	NULL	4	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The stones in 19 of the 23 patients in the multiple stone group remained stable throughout the study , while stones in 4 grew .
	manualset3
166429	1	412622	7	NULL	NULL	0	NULL	storage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The storage of large amounts of data that can help to identify the patient 's allergen microenvironment : -- literature : articles related to contact dermatitis problems ; -- product information such as , for example , the composition of pharmaceutical , cosmetics , and industrial materials ; -- the dermatologist : the filling in of a standardized anamnesis from also helps to assure that relevant clinical data is not overlooked .
	manualset3
166430	2	412622	7	NULL	NULL	0	NULL	large amounts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The storage of large amounts of data that can help to identify the patient 's allergen microenvironment : -- literature : articles related to contact dermatitis problems ; -- product information such as , for example , the composition of pharmaceutical , cosmetics , and industrial materials ; -- the dermatologist : the filling in of a standardized anamnesis from also helps to assure that relevant clinical data is not overlooked .
	manualset3
166431	3	412622	7	NULL	NULL	0	NULL	 data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The storage of large amounts of data that can help to identify the patient 's allergen microenvironment : -- literature : articles related to contact dermatitis problems ; -- product information such as , for example , the composition of pharmaceutical , cosmetics , and industrial materials ; -- the dermatologist : the filling in of a standardized anamnesis from also helps to assure that relevant clinical data is not overlooked .
	manualset3
166432	4	412622	7	NULL	NULL	0	NULL	patient 's allergen microenvironment 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The storage of large amounts of data that can help to identify the patient 's allergen microenvironment : -- literature : articles related to contact dermatitis problems ; -- product information such as , for example , the composition of pharmaceutical , cosmetics , and industrial materials ; -- the dermatologist : the filling in of a standardized anamnesis from also helps to assure that relevant clinical data is not overlooked .
	manualset3
166433	5	412622	7	NULL	NULL	0	NULL	 literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The storage of large amounts of data that can help to identify the patient 's allergen microenvironment : -- literature : articles related to contact dermatitis problems ; -- product information such as , for example , the composition of pharmaceutical , cosmetics , and industrial materials ; -- the dermatologist : the filling in of a standardized anamnesis from also helps to assure that relevant clinical data is not overlooked .
	manualset3
166434	6	412622	7	NULL	NULL	0	NULL	articles	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The storage of large amounts of data that can help to identify the patient 's allergen microenvironment : -- literature : articles related to contact dermatitis problems ; -- product information such as , for example , the composition of pharmaceutical , cosmetics , and industrial materials ; -- the dermatologist : the filling in of a standardized anamnesis from also helps to assure that relevant clinical data is not overlooked .
	manualset3
166435	7	412622	7	NULL	NULL	NULL	NULL	contact dermatitis problems	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The storage of large amounts of data that can help to identify the patient 's allergen microenvironment : -- literature : articles related to contact dermatitis problems ; -- product information such as , for example , the composition of pharmaceutical , cosmetics , and industrial materials ; -- the dermatologist : the filling in of a standardized anamnesis from also helps to assure that relevant clinical data is not overlooked .
	manualset3
166436	8	412622	7	NULL	NULL	0	NULL	product information 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The storage of large amounts of data that can help to identify the patient 's allergen microenvironment : -- literature : articles related to contact dermatitis problems ; -- product information such as , for example , the composition of pharmaceutical , cosmetics , and industrial materials ; -- the dermatologist : the filling in of a standardized anamnesis from also helps to assure that relevant clinical data is not overlooked .
	manualset3
166438	10	412622	7	NULL	NULL	0	NULL	composition 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The storage of large amounts of data that can help to identify the patient 's allergen microenvironment : -- literature : articles related to contact dermatitis problems ; -- product information such as , for example , the composition of pharmaceutical , cosmetics , and industrial materials ; -- the dermatologist : the filling in of a standardized anamnesis from also helps to assure that relevant clinical data is not overlooked .
	manualset3
166439	11	412622	7	NULL	NULL	0	NULL	pharmaceutical materials	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The storage of large amounts of data that can help to identify the patient 's allergen microenvironment : -- literature : articles related to contact dermatitis problems ; -- product information such as , for example , the composition of pharmaceutical , cosmetics , and industrial materials ; -- the dermatologist : the filling in of a standardized anamnesis from also helps to assure that relevant clinical data is not overlooked .
	manualset3
166440	12	412622	7	NULL	NULL	0	NULL	cosmetics materials	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The storage of large amounts of data that can help to identify the patient 's allergen microenvironment : -- literature : articles related to contact dermatitis problems ; -- product information such as , for example , the composition of pharmaceutical , cosmetics , and industrial materials ; -- the dermatologist : the filling in of a standardized anamnesis from also helps to assure that relevant clinical data is not overlooked .
	manualset3
166441	13	412622	7	NULL	NULL	0	NULL	 industrial materials	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The storage of large amounts of data that can help to identify the patient 's allergen microenvironment : -- literature : articles related to contact dermatitis problems ; -- product information such as , for example , the composition of pharmaceutical , cosmetics , and industrial materials ; -- the dermatologist : the filling in of a standardized anamnesis from also helps to assure that relevant clinical data is not overlooked .
	manualset3
166442	14	412622	7	NULL	NULL	0	NULL	dermatologist	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The storage of large amounts of data that can help to identify the patient 's allergen microenvironment : -- literature : articles related to contact dermatitis problems ; -- product information such as , for example , the composition of pharmaceutical , cosmetics , and industrial materials ; -- the dermatologist : the filling in of a standardized anamnesis from also helps to assure that relevant clinical data is not overlooked .
	manualset3
166443	15	412622	7	NULL	NULL	0	NULL	 filling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The storage of large amounts of data that can help to identify the patient 's allergen microenvironment : -- literature : articles related to contact dermatitis problems ; -- product information such as , for example , the composition of pharmaceutical , cosmetics , and industrial materials ; -- the dermatologist : the filling in of a standardized anamnesis from also helps to assure that relevant clinical data is not overlooked .
	manualset3
166444	16	412622	7	NULL	NULL	NULL	NULL	standardized anamnesis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The storage of large amounts of data that can help to identify the patient 's allergen microenvironment : -- literature : articles related to contact dermatitis problems ; -- product information such as , for example , the composition of pharmaceutical , cosmetics , and industrial materials ; -- the dermatologist : the filling in of a standardized anamnesis from also helps to assure that relevant clinical data is not overlooked .
	manualset3
166445	17	412622	7	NULL	NULL	NULL	NULL	clinical data	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The storage of large amounts of data that can help to identify the patient 's allergen microenvironment : -- literature : articles related to contact dermatitis problems ; -- product information such as , for example , the composition of pharmaceutical , cosmetics , and industrial materials ; -- the dermatologist : the filling in of a standardized anamnesis from also helps to assure that relevant clinical data is not overlooked .
	manualset3
166446	1	412623	7	NULL	NULL	0	NULL	strain 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The strain might be practically valuable to prevent diarrhea in calves .
	manualset3
166448	2	412623	7	NULL	NULL	NULL	NULL	diarrhea	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The strain might be practically valuable to prevent diarrhea in calves .
	manualset3
166449	3	412623	7	NULL	NULL	NULL	NULL	calves	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The strain might be practically valuable to prevent diarrhea in calves .
	manualset3
166450	1	412624	7	NULL	NULL	0	NULL	strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The strains were typed by set of 10 experimental phages and compared by the method of PCR-RFLP analysis of coagulase gen restriction fragment length polymorphism .
	manualset3
166451	2	412624	7	NULL	NULL	0	NULL	set	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The strains were typed by set of 10 experimental phages and compared by the method of PCR-RFLP analysis of coagulase gen restriction fragment length polymorphism .
	manualset3
166452	3	412624	7	NULL	NULL	0	NULL	10 experimental phages	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The strains were typed by set of 10 experimental phages and compared by the method of PCR-RFLP analysis of coagulase gen restriction fragment length polymorphism .
	manualset3
166453	4	412624	7	NULL	NULL	0	NULL	 method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The strains were typed by set of 10 experimental phages and compared by the method of PCR-RFLP analysis of coagulase gen restriction fragment length polymorphism .
	manualset3
166454	5	412624	7	NULL	NULL	0	NULL	PCR-RFLP analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The strains were typed by set of 10 experimental phages and compared by the method of PCR-RFLP analysis of coagulase gen restriction fragment length polymorphism .
	manualset3
166455	6	412624	7	NULL	NULL	0	NULL	coagulase gen restriction fragment length polymorphism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The strains were typed by set of 10 experimental phages and compared by the method of PCR-RFLP analysis of coagulase gen restriction fragment length polymorphism .
	manualset3
166456	1	412625	7	NULL	NULL	NULL	NULL	stratified squamous epithelium	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The stratified squamous epithelium covering the lip could be divided into : ( i ) appendage-bearing , orthokeratinised epidermis ; ( ii ) orthokeratinised vermilion which had a more prominent rete pattern than the epidermis ; ( iii ) parakeratinised , PAS-positive intermediate zone ; and ( iv ) non - or parakeratinised labial mucosal epithelium .
	manualset3
166457	2	412625	7	NULL	NULL	0	NULL	lip	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The stratified squamous epithelium covering the lip could be divided into : ( i ) appendage-bearing , orthokeratinised epidermis ; ( ii ) orthokeratinised vermilion which had a more prominent rete pattern than the epidermis ; ( iii ) parakeratinised , PAS-positive intermediate zone ; and ( iv ) non - or parakeratinised labial mucosal epithelium .
	manualset3
166458	3	412625	7	NULL	NULL	NULL	NULL	 appendage-bearing , orthokeratinised epidermis 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The stratified squamous epithelium covering the lip could be divided into : ( i ) appendage-bearing , orthokeratinised epidermis ; ( ii ) orthokeratinised vermilion which had a more prominent rete pattern than the epidermis ; ( iii ) parakeratinised , PAS-positive intermediate zone ; and ( iv ) non - or parakeratinised labial mucosal epithelium .
	manualset3
166459	4	412625	7	NULL	NULL	0	NULL	orthokeratinised vermilion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The stratified squamous epithelium covering the lip could be divided into : ( i ) appendage-bearing , orthokeratinised epidermis ; ( ii ) orthokeratinised vermilion which had a more prominent rete pattern than the epidermis ; ( iii ) parakeratinised , PAS-positive intermediate zone ; and ( iv ) non - or parakeratinised labial mucosal epithelium .
	manualset3
166460	5	412625	7	NULL	NULL	0	NULL	rete pattern	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The stratified squamous epithelium covering the lip could be divided into : ( i ) appendage-bearing , orthokeratinised epidermis ; ( ii ) orthokeratinised vermilion which had a more prominent rete pattern than the epidermis ; ( iii ) parakeratinised , PAS-positive intermediate zone ; and ( iv ) non - or parakeratinised labial mucosal epithelium .
	manualset3
166461	6	412625	7	NULL	NULL	NULL	NULL	epidermis	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The stratified squamous epithelium covering the lip could be divided into : ( i ) appendage-bearing , orthokeratinised epidermis ; ( ii ) orthokeratinised vermilion which had a more prominent rete pattern than the epidermis ; ( iii ) parakeratinised , PAS-positive intermediate zone ; and ( iv ) non - or parakeratinised labial mucosal epithelium .
	manualset3
166462	7	412625	7	NULL	NULL	0	NULL	 parakeratinised , PAS-positive intermediate zone	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The stratified squamous epithelium covering the lip could be divided into : ( i ) appendage-bearing , orthokeratinised epidermis ; ( ii ) orthokeratinised vermilion which had a more prominent rete pattern than the epidermis ; ( iii ) parakeratinised , PAS-positive intermediate zone ; and ( iv ) non - or parakeratinised labial mucosal epithelium .
	manualset3
166463	8	412625	7	NULL	NULL	NULL	NULL	non - or parakeratinised labial mucosal epithelium	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The stratified squamous epithelium covering the lip could be divided into : ( i ) appendage-bearing , orthokeratinised epidermis ; ( ii ) orthokeratinised vermilion which had a more prominent rete pattern than the epidermis ; ( iii ) parakeratinised , PAS-positive intermediate zone ; and ( iv ) non - or parakeratinised labial mucosal epithelium .
	manualset3
166464	1	412626	7	NULL	NULL	NULL	NULL	evidence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Accumulating evidence suggests that the therapeutic margin of aminoglycoside therapy may be improved by manipulation of dosing strategy .
	manualset3
166465	2	412626	7	NULL	NULL	0	NULL	therapeutic margin	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Accumulating evidence suggests that the therapeutic margin of aminoglycoside therapy may be improved by manipulation of dosing strategy .
	manualset3
166466	3	412626	7	NULL	NULL	0	NULL	aminoglycoside therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Accumulating evidence suggests that the therapeutic margin of aminoglycoside therapy may be improved by manipulation of dosing strategy .
	manualset3
166467	4	412626	7	NULL	NULL	0	NULL	manipulation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Accumulating evidence suggests that the therapeutic margin of aminoglycoside therapy may be improved by manipulation of dosing strategy .
	manualset3
166468	5	412626	7	NULL	NULL	0	NULL	dosing strategy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Accumulating evidence suggests that the therapeutic margin of aminoglycoside therapy may be improved by manipulation of dosing strategy .
	manualset3
166469	1	412627	7	NULL	NULL	0	NULL	stratopause	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The stratopause height increases from 0.1 mbar near the equator to 0.01 mbar near the North Pole , where it is the warmest part of the atmosphere , greater than 200K .
	manualset3
166470	2	412627	7	NULL	NULL	0	NULL	height	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The stratopause height increases from 0.1 mbar near the equator to 0.01 mbar near the North Pole , where it is the warmest part of the atmosphere , greater than 200K .
	manualset3
166471	3	412627	7	NULL	NULL	0	NULL	0.1 mbar	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The stratopause height increases from 0.1 mbar near the equator to 0.01 mbar near the North Pole , where it is the warmest part of the atmosphere , greater than 200K .
	manualset3
166472	4	412627	7	NULL	NULL	0	NULL	equator	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The stratopause height increases from 0.1 mbar near the equator to 0.01 mbar near the North Pole , where it is the warmest part of the atmosphere , greater than 200K .
	manualset3
166473	5	412627	7	NULL	NULL	0	NULL	0.01 mbar	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The stratopause height increases from 0.1 mbar near the equator to 0.01 mbar near the North Pole , where it is the warmest part of the atmosphere , greater than 200K .
	manualset3
166474	6	412627	7	NULL	NULL	0	NULL	North Pole	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The stratopause height increases from 0.1 mbar near the equator to 0.01 mbar near the North Pole , where it is the warmest part of the atmosphere , greater than 200K .
	manualset3
166475	7	412627	7	NULL	NULL	0	NULL	warmest part	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The stratopause height increases from 0.1 mbar near the equator to 0.01 mbar near the North Pole , where it is the warmest part of the atmosphere , greater than 200K .
	manualset3
166476	8	412627	7	NULL	NULL	0	NULL	atmosphere	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The stratopause height increases from 0.1 mbar near the equator to 0.01 mbar near the North Pole , where it is the warmest part of the atmosphere , greater than 200K .
	manualset3
166477	9	412627	7	NULL	NULL	0	NULL	200K	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The stratopause height increases from 0.1 mbar near the equator to 0.01 mbar near the North Pole , where it is the warmest part of the atmosphere , greater than 200K .
	manualset3
166478	1	412628	7	NULL	NULL	0	NULL	strength	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The strength of B cell antigen receptor ( BCR ) signaling in response to antigen increases with affinity , a process known as `` affinity discrimination '' .
	manualset3
166479	2	412628	7	NULL	NULL	0	NULL	B cell antigen receptor ( BCR ) signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The strength of B cell antigen receptor ( BCR ) signaling in response to antigen increases with affinity , a process known as `` affinity discrimination '' .
	manualset3
166480	3	412628	7	NULL	NULL	0	NULL	response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The strength of B cell antigen receptor ( BCR ) signaling in response to antigen increases with affinity , a process known as `` affinity discrimination '' .
	manualset3
166481	4	412628	7	NULL	NULL	0	NULL	antigen	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The strength of B cell antigen receptor ( BCR ) signaling in response to antigen increases with affinity , a process known as `` affinity discrimination '' .
	manualset3
166482	5	412628	7	NULL	NULL	0	NULL	affinity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The strength of B cell antigen receptor ( BCR ) signaling in response to antigen increases with affinity , a process known as `` affinity discrimination '' .
	manualset3
166483	6	412628	7	NULL	NULL	0	NULL	process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The strength of B cell antigen receptor ( BCR ) signaling in response to antigen increases with affinity , a process known as `` affinity discrimination '' .
	manualset3
166484	7	412628	7	NULL	NULL	0	NULL	affinity discrimination	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The strength of B cell antigen receptor ( BCR ) signaling in response to antigen increases with affinity , a process known as `` affinity discrimination '' .
	manualset3
166485	1	412629	7	NULL	NULL	0	NULL	stretch-activated ANP secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The stretch-activated ANP secretion was suppressed without significant difference in basal ANP secretion , as compared to control right atria .
	manualset3
166486	2	412629	7	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The stretch-activated ANP secretion was suppressed without significant difference in basal ANP secretion , as compared to control right atria .
	manualset3
166487	3	412629	7	NULL	NULL	0	NULL	basal ANP secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The stretch-activated ANP secretion was suppressed without significant difference in basal ANP secretion , as compared to control right atria .
	manualset3
166488	4	412629	7	NULL	NULL	0	NULL	 right atria	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The stretch-activated ANP secretion was suppressed without significant difference in basal ANP secretion , as compared to control right atria .
	manualset3
166489	1	412630	7	NULL	NULL	NULL	NULL	 strong adsorption	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The strong adsorption of ammonia caused by chemical interactions on different adsorption sites is evidenced by the trends in the isosteric heats of adsorption .
	manualset3
166490	3	412630	7	NULL	NULL	NULL	NULL	chemical interactions 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The strong adsorption of ammonia caused by chemical interactions on different adsorption sites is evidenced by the trends in the isosteric heats of adsorption .
	manualset3
166491	4	412630	7	NULL	NULL	NULL	NULL	adsorption sites	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The strong adsorption of ammonia caused by chemical interactions on different adsorption sites is evidenced by the trends in the isosteric heats of adsorption .
	manualset3
166492	5	412630	7	NULL	NULL	NULL	NULL	 trends	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The strong adsorption of ammonia caused by chemical interactions on different adsorption sites is evidenced by the trends in the isosteric heats of adsorption .
	manualset3
166493	6	412630	7	NULL	NULL	NULL	NULL	isosteric heats of adsorption	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The strong adsorption of ammonia caused by chemical interactions on different adsorption sites is evidenced by the trends in the isosteric heats of adsorption .
	manualset3
166513	2	412630	7	NULL	NULL	0	NULL	ammonia	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The strong adsorption of ammonia caused by chemical interactions on different adsorption sites is evidenced by the trends in the isosteric heats of adsorption .
	manualset3
166514	1	412631	7	NULL	NULL	0	NULL	strong potentiation effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The strong potentiation effect of ascorbic acid was reproduced using apomorphine .
	manualset3
166515	2	412631	7	NULL	NULL	0	NULL	ascorbic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The strong potentiation effect of ascorbic acid was reproduced using apomorphine .
	manualset3
166516	3	412631	7	NULL	NULL	0	NULL	apomorphine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The strong potentiation effect of ascorbic acid was reproduced using apomorphine .
	manualset3
166517	1	412632	7	NULL	NULL	0	NULL	strong relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The strong relation of central fat to insulin response was noted in both races and sexes but not in either sexually immature or relatively thin children .
	manualset3
166518	2	412632	7	NULL	NULL	0	NULL	 central fat	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The strong relation of central fat to insulin response was noted in both races and sexes but not in either sexually immature or relatively thin children .
	manualset3
166519	3	412632	7	NULL	NULL	NULL	NULL	 insulin response	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The strong relation of central fat to insulin response was noted in both races and sexes but not in either sexually immature or relatively thin children .
	manualset3
166520	4	412632	7	NULL	NULL	0	NULL	races 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The strong relation of central fat to insulin response was noted in both races and sexes but not in either sexually immature or relatively thin children .
	manualset3
166521	5	412632	7	NULL	NULL	0	NULL	sexes	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The strong relation of central fat to insulin response was noted in both races and sexes but not in either sexually immature or relatively thin children .
	manualset3
166522	6	412632	7	NULL	NULL	0	NULL	sexually immature children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The strong relation of central fat to insulin response was noted in both races and sexes but not in either sexually immature or relatively thin children .
	manualset3
166523	7	412632	7	NULL	NULL	0	NULL	relatively thin children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The strong relation of central fat to insulin response was noted in both races and sexes but not in either sexually immature or relatively thin children .
	manualset3
166524	1	412633	7	NULL	NULL	0	NULL	strongest association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The strongest association was with diabetic nephropathy , but two - to three-fold risk elevations were observed for all major subtypes of CRF .
	manualset3
166525	2	412633	7	NULL	NULL	0	NULL	diabetic nephropathy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The strongest association was with diabetic nephropathy , but two - to three-fold risk elevations were observed for all major subtypes of CRF .
	manualset3
166526	3	412633	7	NULL	NULL	0	NULL	two - to three-fold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The strongest association was with diabetic nephropathy , but two - to three-fold risk elevations were observed for all major subtypes of CRF .
	manualset3
166527	4	412633	7	NULL	NULL	0	NULL	risk elevations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The strongest association was with diabetic nephropathy , but two - to three-fold risk elevations were observed for all major subtypes of CRF .
	manualset3
166528	5	412633	7	NULL	NULL	0	NULL	major subtypes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The strongest association was with diabetic nephropathy , but two - to three-fold risk elevations were observed for all major subtypes of CRF .
	manualset3
166529	6	412633	7	NULL	NULL	0	NULL	CRF	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The strongest association was with diabetic nephropathy , but two - to three-fold risk elevations were observed for all major subtypes of CRF .
	manualset3
166530	1	412634	7	NULL	NULL	0	NULL	strongest evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The strongest evidence in support of a developmental trend was seen in definitions of illness pertaining to changes in daily activities .
	manualset3
166531	2	412634	7	NULL	NULL	0	NULL	support 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The strongest evidence in support of a developmental trend was seen in definitions of illness pertaining to changes in daily activities .
	manualset3
166532	3	412634	7	NULL	NULL	0	NULL	definitions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The strongest evidence in support of a developmental trend was seen in definitions of illness pertaining to changes in daily activities .
	manualset3
166533	4	412634	7	NULL	NULL	0	NULL	illness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The strongest evidence in support of a developmental trend was seen in definitions of illness pertaining to changes in daily activities .
	manualset3
166534	5	412634	7	NULL	NULL	0	NULL	daily activities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The strongest evidence in support of a developmental trend was seen in definitions of illness pertaining to changes in daily activities .
	manualset3
166535	1	412635	7	NULL	NULL	0	NULL	structural characterization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural characterization of 3 revealed a ( Au ( CN ) ( 2 ) ) ( - ) / pyz-based framework similar to previously reported Cu ( pyz ) ( Au ( CN ) ( 2 ) ) ( 2 ) , whereas 7 formed an intricate network consisting of individual 2-D networks held together by AuAu interactions and featuring the rare ( AuBrCN ) ( - ) unit .
	manualset3
166536	2	412635	7	NULL	NULL	0	NULL	3	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural characterization of 3 revealed a ( Au ( CN ) ( 2 ) ) ( - ) / pyz-based framework similar to previously reported Cu ( pyz ) ( Au ( CN ) ( 2 ) ) ( 2 ) , whereas 7 formed an intricate network consisting of individual 2-D networks held together by AuAu interactions and featuring the rare ( AuBrCN ) ( - ) unit .
	manualset3
166537	3	412635	7	NULL	NULL	0	NULL	( Au ( CN ) ( 2 ) ) ( - ) / pyz-based framework	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural characterization of 3 revealed a ( Au ( CN ) ( 2 ) ) ( - ) / pyz-based framework similar to previously reported Cu ( pyz ) ( Au ( CN ) ( 2 ) ) ( 2 ) , whereas 7 formed an intricate network consisting of individual 2-D networks held together by AuAu interactions and featuring the rare ( AuBrCN ) ( - ) unit .
	manualset3
166538	4	412635	7	NULL	NULL	0	NULL	similar	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural characterization of 3 revealed a ( Au ( CN ) ( 2 ) ) ( - ) / pyz-based framework similar to previously reported Cu ( pyz ) ( Au ( CN ) ( 2 ) ) ( 2 ) , whereas 7 formed an intricate network consisting of individual 2-D networks held together by AuAu interactions and featuring the rare ( AuBrCN ) ( - ) unit .
	manualset3
166539	5	412635	7	NULL	NULL	0	NULL	Cu ( pyz ) ( Au ( CN ) ( 2 ) ) ( 2 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural characterization of 3 revealed a ( Au ( CN ) ( 2 ) ) ( - ) / pyz-based framework similar to previously reported Cu ( pyz ) ( Au ( CN ) ( 2 ) ) ( 2 ) , whereas 7 formed an intricate network consisting of individual 2-D networks held together by AuAu interactions and featuring the rare ( AuBrCN ) ( - ) unit .
	manualset3
166540	6	412635	7	NULL	NULL	0	NULL	 7	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural characterization of 3 revealed a ( Au ( CN ) ( 2 ) ) ( - ) / pyz-based framework similar to previously reported Cu ( pyz ) ( Au ( CN ) ( 2 ) ) ( 2 ) , whereas 7 formed an intricate network consisting of individual 2-D networks held together by AuAu interactions and featuring the rare ( AuBrCN ) ( - ) unit .
	manualset3
166541	7	412635	7	NULL	NULL	NULL	NULL	intricate network	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The structural characterization of 3 revealed a ( Au ( CN ) ( 2 ) ) ( - ) / pyz-based framework similar to previously reported Cu ( pyz ) ( Au ( CN ) ( 2 ) ) ( 2 ) , whereas 7 formed an intricate network consisting of individual 2-D networks held together by AuAu interactions and featuring the rare ( AuBrCN ) ( - ) unit .
	manualset3
166542	8	412635	7	NULL	NULL	0	NULL	individual 2-D networks	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural characterization of 3 revealed a ( Au ( CN ) ( 2 ) ) ( - ) / pyz-based framework similar to previously reported Cu ( pyz ) ( Au ( CN ) ( 2 ) ) ( 2 ) , whereas 7 formed an intricate network consisting of individual 2-D networks held together by AuAu interactions and featuring the rare ( AuBrCN ) ( - ) unit .
	manualset3
166543	9	412635	7	NULL	NULL	0	NULL	AuAu interactions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural characterization of 3 revealed a ( Au ( CN ) ( 2 ) ) ( - ) / pyz-based framework similar to previously reported Cu ( pyz ) ( Au ( CN ) ( 2 ) ) ( 2 ) , whereas 7 formed an intricate network consisting of individual 2-D networks held together by AuAu interactions and featuring the rare ( AuBrCN ) ( - ) unit .
	manualset3
166544	10	412635	7	NULL	NULL	0	NULL	rare ( AuBrCN ) ( - ) unit 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural characterization of 3 revealed a ( Au ( CN ) ( 2 ) ) ( - ) / pyz-based framework similar to previously reported Cu ( pyz ) ( Au ( CN ) ( 2 ) ) ( 2 ) , whereas 7 formed an intricate network consisting of individual 2-D networks held together by AuAu interactions and featuring the rare ( AuBrCN ) ( - ) unit .
	manualset3
166545	1	412636	7	NULL	NULL	0	NULL	Accumulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Accumulation of these cells was most prominent at day 12 within the granulation tissues and they were still present in fibrotic areas between days 12 and 24 and diminished markedly afterward .
	manualset3
166546	2	412636	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Accumulation of these cells was most prominent at day 12 within the granulation tissues and they were still present in fibrotic areas between days 12 and 24 and diminished markedly afterward .
	manualset3
166547	3	412636	7	NULL	NULL	0	NULL	 day 12	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Accumulation of these cells was most prominent at day 12 within the granulation tissues and they were still present in fibrotic areas between days 12 and 24 and diminished markedly afterward .
	manualset3
166548	4	412636	7	NULL	NULL	0	NULL	granulation tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Accumulation of these cells was most prominent at day 12 within the granulation tissues and they were still present in fibrotic areas between days 12 and 24 and diminished markedly afterward .
	manualset3
166549	5	412636	7	NULL	NULL	0	NULL	fibrotic areas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Accumulation of these cells was most prominent at day 12 within the granulation tissues and they were still present in fibrotic areas between days 12 and 24 and diminished markedly afterward .
	manualset3
166550	6	412636	7	NULL	NULL	0	NULL	days 12 and 24	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Accumulation of these cells was most prominent at day 12 within the granulation tissues and they were still present in fibrotic areas between days 12 and 24 and diminished markedly afterward .
	manualset3
166551	1	412637	7	NULL	NULL	0	NULL	structural determinants	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural determinants that support the affinity and selectivity profiles of the series were highlighted through an integrated computational approach , combining a 3D-QSAR model built on the second generation of GRid INdependent Descriptors ( GRIND2 ) with a novel homology model of the hA ( 3 ) receptor .
	manualset3
166552	2	412637	7	NULL	NULL	0	NULL	affinity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural determinants that support the affinity and selectivity profiles of the series were highlighted through an integrated computational approach , combining a 3D-QSAR model built on the second generation of GRid INdependent Descriptors ( GRIND2 ) with a novel homology model of the hA ( 3 ) receptor .
	manualset3
166553	3	412637	7	NULL	NULL	0	NULL	 selectivity profiles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural determinants that support the affinity and selectivity profiles of the series were highlighted through an integrated computational approach , combining a 3D-QSAR model built on the second generation of GRid INdependent Descriptors ( GRIND2 ) with a novel homology model of the hA ( 3 ) receptor .
	manualset3
166554	4	412637	7	NULL	NULL	0	NULL	 series 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural determinants that support the affinity and selectivity profiles of the series were highlighted through an integrated computational approach , combining a 3D-QSAR model built on the second generation of GRid INdependent Descriptors ( GRIND2 ) with a novel homology model of the hA ( 3 ) receptor .
	manualset3
166555	5	412637	7	NULL	NULL	0	NULL	integrated computational approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural determinants that support the affinity and selectivity profiles of the series were highlighted through an integrated computational approach , combining a 3D-QSAR model built on the second generation of GRid INdependent Descriptors ( GRIND2 ) with a novel homology model of the hA ( 3 ) receptor .
	manualset3
166556	6	412637	7	NULL	NULL	0	NULL	3D-QSAR model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural determinants that support the affinity and selectivity profiles of the series were highlighted through an integrated computational approach , combining a 3D-QSAR model built on the second generation of GRid INdependent Descriptors ( GRIND2 ) with a novel homology model of the hA ( 3 ) receptor .
	manualset3
166557	7	412637	7	NULL	NULL	NULL	NULL	 second generation 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The structural determinants that support the affinity and selectivity profiles of the series were highlighted through an integrated computational approach , combining a 3D-QSAR model built on the second generation of GRid INdependent Descriptors ( GRIND2 ) with a novel homology model of the hA ( 3 ) receptor .
	manualset3
166558	8	412637	7	NULL	NULL	NULL	NULL	GRid INdependent Descriptors ( GRIND2 )	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The structural determinants that support the affinity and selectivity profiles of the series were highlighted through an integrated computational approach , combining a 3D-QSAR model built on the second generation of GRid INdependent Descriptors ( GRIND2 ) with a novel homology model of the hA ( 3 ) receptor .
	manualset3
166559	9	412637	7	NULL	NULL	0	NULL	novel homology model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural determinants that support the affinity and selectivity profiles of the series were highlighted through an integrated computational approach , combining a 3D-QSAR model built on the second generation of GRid INdependent Descriptors ( GRIND2 ) with a novel homology model of the hA ( 3 ) receptor .
	manualset3
166560	10	412637	7	NULL	NULL	0	NULL	hA ( 3 ) receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural determinants that support the affinity and selectivity profiles of the series were highlighted through an integrated computational approach , combining a 3D-QSAR model built on the second generation of GRid INdependent Descriptors ( GRIND2 ) with a novel homology model of the hA ( 3 ) receptor .
	manualset3
166562	1	412638	7	NULL	NULL	0	NULL	structural diversity	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural diversity of 1a and 2a resulted in different electronic effects of nitro-group on Pc rings , which caused them have two kinds of Q bands .
	manualset3
166563	2	412638	7	NULL	NULL	0	NULL	1a	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural diversity of 1a and 2a resulted in different electronic effects of nitro-group on Pc rings , which caused them have two kinds of Q bands .
	manualset3
166564	3	412638	7	NULL	NULL	0	NULL	2a	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural diversity of 1a and 2a resulted in different electronic effects of nitro-group on Pc rings , which caused them have two kinds of Q bands .
	manualset3
166565	4	412638	7	NULL	NULL	0	NULL	electronic effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural diversity of 1a and 2a resulted in different electronic effects of nitro-group on Pc rings , which caused them have two kinds of Q bands .
	manualset3
166566	5	412638	7	NULL	NULL	0	NULL	nitro-group on Pc rings	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural diversity of 1a and 2a resulted in different electronic effects of nitro-group on Pc rings , which caused them have two kinds of Q bands .
	manualset3
166567	6	412638	7	NULL	NULL	0	NULL	two kinds	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural diversity of 1a and 2a resulted in different electronic effects of nitro-group on Pc rings , which caused them have two kinds of Q bands .
	manualset3
166568	7	412638	7	NULL	NULL	0	NULL	Q bands	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural diversity of 1a and 2a resulted in different electronic effects of nitro-group on Pc rings , which caused them have two kinds of Q bands .
	manualset3
166569	1	412639	7	NULL	NULL	0	NULL	structure-based design	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure-based design , synthesis , and biological activity of a novel indazole-containing inhibitor series for S-adenosyl homocysteine/methylthioadenosine ( SAH/MTA ) nucleosidase are described .
	manualset3
166570	2	412639	7	NULL	NULL	0	NULL	synthesis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure-based design , synthesis , and biological activity of a novel indazole-containing inhibitor series for S-adenosyl homocysteine/methylthioadenosine ( SAH/MTA ) nucleosidase are described .
	manualset3
166571	3	412639	7	NULL	NULL	NULL	NULL	biological activity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The structure-based design , synthesis , and biological activity of a novel indazole-containing inhibitor series for S-adenosyl homocysteine/methylthioadenosine ( SAH/MTA ) nucleosidase are described .
	manualset3
166572	4	412639	7	NULL	NULL	0	NULL	novel indazole-containing inhibitor series	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure-based design , synthesis , and biological activity of a novel indazole-containing inhibitor series for S-adenosyl homocysteine/methylthioadenosine ( SAH/MTA ) nucleosidase are described .
	manualset3
166573	5	412639	7	NULL	NULL	0	NULL	S-adenosyl homocysteine/methylthioadenosine ( SAH/MTA ) nucleosidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure-based design , synthesis , and biological activity of a novel indazole-containing inhibitor series for S-adenosyl homocysteine/methylthioadenosine ( SAH/MTA ) nucleosidase are described .
	manualset3
166574	1	412640	7	NULL	NULL	0	NULL	 structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure and the function of interphase AgNORs and the importance of the `` AgNOR '' parameter in tumor pathology have been reviewed .
	manualset3
166575	2	412640	7	NULL	NULL	0	NULL	function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure and the function of interphase AgNORs and the importance of the `` AgNOR '' parameter in tumor pathology have been reviewed .
	manualset3
166576	3	412640	7	NULL	NULL	0	NULL	interphase AgNORs 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure and the function of interphase AgNORs and the importance of the `` AgNOR '' parameter in tumor pathology have been reviewed .
	manualset3
166577	4	412640	7	NULL	NULL	0	NULL	importance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure and the function of interphase AgNORs and the importance of the `` AgNOR '' parameter in tumor pathology have been reviewed .
	manualset3
166578	5	412640	7	NULL	NULL	NULL	NULL	`` AgNOR '' parameter	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The structure and the function of interphase AgNORs and the importance of the `` AgNOR '' parameter in tumor pathology have been reviewed .
	manualset3
166579	6	412640	7	NULL	NULL	0	NULL	tumor pathology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure and the function of interphase AgNORs and the importance of the `` AgNOR '' parameter in tumor pathology have been reviewed .
	manualset3
166580	1	412641	7	NULL	NULL	0	NULL	 structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure displays a peculiar stereochemistry of the cation .
	manualset3
166581	2	412641	7	NULL	NULL	0	NULL	stereochemistry	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure displays a peculiar stereochemistry of the cation .
	manualset3
166582	3	412641	7	NULL	NULL	0	NULL	cation	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure displays a peculiar stereochemistry of the cation .
	manualset3
166583	1	412642	7	NULL	NULL	0	NULL	structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure identifies variable residues that likely mediate discrimination between lysine - and diaminopimelic acid-type PGNs .
	manualset3
166584	2	412642	7	NULL	NULL	0	NULL	 variable residues	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure identifies variable residues that likely mediate discrimination between lysine - and diaminopimelic acid-type PGNs .
	manualset3
166585	3	412642	7	NULL	NULL	0	NULL	discrimination	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure identifies variable residues that likely mediate discrimination between lysine - and diaminopimelic acid-type PGNs .
	manualset3
166586	4	412642	7	NULL	NULL	0	NULL	lysine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure identifies variable residues that likely mediate discrimination between lysine - and diaminopimelic acid-type PGNs .
	manualset3
166587	5	412642	7	NULL	NULL	0	NULL	diaminopimelic acid-type PGNs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure identifies variable residues that likely mediate discrimination between lysine - and diaminopimelic acid-type PGNs .
	manualset3
166588	1	412643	7	NULL	NULL	0	NULL	 structure 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure is well-defined except for N-terminal residues 4-6 and C-terminal residues 67-72 .
	manualset3
166589	2	412643	7	NULL	NULL	0	NULL	N-terminal residues 4-6	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure is well-defined except for N-terminal residues 4-6 and C-terminal residues 67-72 .
	manualset3
166590	3	412643	7	NULL	NULL	0	NULL	C-terminal residues 67-72	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure is well-defined except for N-terminal residues 4-6 and C-terminal residues 67-72 .
	manualset3
166591	1	412644	7	NULL	NULL	0	NULL	Accuracy 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Accuracy of AJCC staging for breast cancer patients undergoing re-excision for positive margins .
	manualset3
166592	2	412644	7	NULL	NULL	0	NULL	AJCC staging	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Accuracy of AJCC staging for breast cancer patients undergoing re-excision for positive margins .
	manualset3
166593	3	412644	7	NULL	NULL	0	NULL	breast cancer patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Accuracy of AJCC staging for breast cancer patients undergoing re-excision for positive margins .
	manualset3
166594	4	412644	7	NULL	NULL	0	NULL	 re-excision	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Accuracy of AJCC staging for breast cancer patients undergoing re-excision for positive margins .
	manualset3
166595	5	412644	7	NULL	NULL	0	NULL	positive margins	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Accuracy of AJCC staging for breast cancer patients undergoing re-excision for positive margins .
	manualset3
166596	1	412645	7	NULL	NULL	0	NULL	 structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of JNK3 in complex with small molecule inhibitors : structural basis for potency and selectivity .
	manualset3
166597	2	412645	7	NULL	NULL	0	NULL	JNK3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of JNK3 in complex with small molecule inhibitors : structural basis for potency and selectivity .
	manualset3
166598	3	412645	7	NULL	NULL	0	NULL	complex	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of JNK3 in complex with small molecule inhibitors : structural basis for potency and selectivity .
	manualset3
166599	4	412645	7	NULL	NULL	0	NULL	small molecule inhibitors	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of JNK3 in complex with small molecule inhibitors : structural basis for potency and selectivity .
	manualset3
166600	5	412645	7	NULL	NULL	0	NULL	structural basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of JNK3 in complex with small molecule inhibitors : structural basis for potency and selectivity .
	manualset3
166601	6	412645	7	NULL	NULL	0	NULL	potency 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of JNK3 in complex with small molecule inhibitors : structural basis for potency and selectivity .
	manualset3
166602	7	412645	7	NULL	NULL	0	NULL	selectivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of JNK3 in complex with small molecule inhibitors : structural basis for potency and selectivity .
	manualset3
166603	1	412646	7	NULL	NULL	0	NULL	 structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of pore complexes reconstructed in the absence of protein synthesis can not be distinguished from the structure of those of control cells .
	manualset3
166604	2	412646	7	NULL	NULL	0	NULL	pore complexes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of pore complexes reconstructed in the absence of protein synthesis can not be distinguished from the structure of those of control cells .
	manualset3
166605	3	412646	7	NULL	NULL	0	NULL	absence	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of pore complexes reconstructed in the absence of protein synthesis can not be distinguished from the structure of those of control cells .
	manualset3
166606	4	412646	7	NULL	NULL	0	NULL	protein synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of pore complexes reconstructed in the absence of protein synthesis can not be distinguished from the structure of those of control cells .
	manualset3
166607	5	412646	7	NULL	NULL	0	NULL	structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of pore complexes reconstructed in the absence of protein synthesis can not be distinguished from the structure of those of control cells .
	manualset3
166608	6	412646	7	NULL	NULL	0	NULL	control cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of pore complexes reconstructed in the absence of protein synthesis can not be distinguished from the structure of those of control cells .
	manualset3
166609	1	412647	7	NULL	NULL	0	NULL	structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of program evaluation : an approach for evaluating a course , clerkship , or components of a residency or fellowship training program .
	manualset3
166610	2	412647	7	NULL	NULL	0	NULL	program evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of program evaluation : an approach for evaluating a course , clerkship , or components of a residency or fellowship training program .
	manualset3
166611	3	412647	7	NULL	NULL	0	NULL	approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of program evaluation : an approach for evaluating a course , clerkship , or components of a residency or fellowship training program .
	manualset3
166612	4	412647	7	NULL	NULL	0	NULL	course	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of program evaluation : an approach for evaluating a course , clerkship , or components of a residency or fellowship training program .
	manualset3
166613	5	412647	7	NULL	NULL	0	NULL	clerkship	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of program evaluation : an approach for evaluating a course , clerkship , or components of a residency or fellowship training program .
	manualset3
166614	6	412647	7	NULL	NULL	0	NULL	components 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of program evaluation : an approach for evaluating a course , clerkship , or components of a residency or fellowship training program .
	manualset3
166615	7	412647	7	NULL	NULL	0	NULL	residency training program	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of program evaluation : an approach for evaluating a course , clerkship , or components of a residency or fellowship training program .
	manualset3
166616	8	412647	7	NULL	NULL	0	NULL	fellowship training program	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of program evaluation : an approach for evaluating a course , clerkship , or components of a residency or fellowship training program .
	manualset3
166617	1	412648	7	NULL	NULL	0	NULL	structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of the Gla-domainless form of the human anticoagulant enzyme activated protein C has been solved at 2.8 A resolution .
	manualset3
166618	2	412648	7	NULL	NULL	0	NULL	Gla-domainless form 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of the Gla-domainless form of the human anticoagulant enzyme activated protein C has been solved at 2.8 A resolution .
	manualset3
166619	3	412648	7	NULL	NULL	0	NULL	human anticoagulant enzyme activated protein C	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of the Gla-domainless form of the human anticoagulant enzyme activated protein C has been solved at 2.8 A resolution .
	manualset3
166620	4	412648	7	NULL	NULL	0	NULL	2.8 A resolution	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of the Gla-domainless form of the human anticoagulant enzyme activated protein C has been solved at 2.8 A resolution .
	manualset3
166621	1	412649	7	NULL	NULL	0	NULL	structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of the eye-ball of Rhimomugil corsula has been described .
	manualset3
166622	2	412649	7	NULL	NULL	0	NULL	 eye-ball	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of the eye-ball of Rhimomugil corsula has been described .
	manualset3
166623	3	412649	7	NULL	NULL	0	NULL	Rhimomugil corsula 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of the eye-ball of Rhimomugil corsula has been described .
	manualset3
166624	1	412650	7	NULL	NULL	0	NULL	structure 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of the title compound , pentoxifylline , C ( 13 ) H ( 18 ) N ( 4 ) O ( 3 ) , has been previously characterized as a triclinic polymorph ( Pavelk et al. ( 1989 ) .
	manualset3
166625	2	412650	7	NULL	NULL	0	NULL	 title compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of the title compound , pentoxifylline , C ( 13 ) H ( 18 ) N ( 4 ) O ( 3 ) , has been previously characterized as a triclinic polymorph ( Pavelk et al. ( 1989 ) .
	manualset3
166626	3	412650	7	NULL	NULL	0	NULL	pentoxifylline , C ( 13 ) H ( 18 ) N ( 4 ) O ( 3 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of the title compound , pentoxifylline , C ( 13 ) H ( 18 ) N ( 4 ) O ( 3 ) , has been previously characterized as a triclinic polymorph ( Pavelk et al. ( 1989 ) .
	manualset3
166627	4	412650	7	NULL	NULL	0	NULL	triclinic polymorph 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of the title compound , pentoxifylline , C ( 13 ) H ( 18 ) N ( 4 ) O ( 3 ) , has been previously characterized as a triclinic polymorph ( Pavelk et al. ( 1989 ) .
	manualset3
166628	5	412650	7	NULL	NULL	0	NULL	Pavelk et al.	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure of the title compound , pentoxifylline , C ( 13 ) H ( 18 ) N ( 4 ) O ( 3 ) , has been previously characterized as a triclinic polymorph ( Pavelk et al. ( 1989 ) .
	manualset3
166629	6	412650	7	NULL	NULL	NULL	NULL	1989	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The structure of the title compound , pentoxifylline , C ( 13 ) H ( 18 ) N ( 4 ) O ( 3 ) , has been previously characterized as a triclinic polymorph ( Pavelk et al. ( 1989 ) .
	manualset3
166630	1	412651	7	NULL	NULL	0	NULL	Accuracy	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Accuracy was the best at 75.1 % for Virga in stage 3 , while it was the highest of 70.7 % for MDRD2-IDMS in stage 4 .
	manualset3
166631	2	412651	7	NULL	NULL	0	NULL	75.1 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Accuracy was the best at 75.1 % for Virga in stage 3 , while it was the highest of 70.7 % for MDRD2-IDMS in stage 4 .
	manualset3
166632	3	412651	7	NULL	NULL	0	NULL	Virga	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Accuracy was the best at 75.1 % for Virga in stage 3 , while it was the highest of 70.7 % for MDRD2-IDMS in stage 4 .
	manualset3
166633	4	412651	7	NULL	NULL	0	NULL	stage 3	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Accuracy was the best at 75.1 % for Virga in stage 3 , while it was the highest of 70.7 % for MDRD2-IDMS in stage 4 .
	manualset3
166634	5	412651	7	NULL	NULL	0	NULL	70.7 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Accuracy was the best at 75.1 % for Virga in stage 3 , while it was the highest of 70.7 % for MDRD2-IDMS in stage 4 .
	manualset3
166635	6	412651	7	NULL	NULL	0	NULL	MDRD2-IDMS	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Accuracy was the best at 75.1 % for Virga in stage 3 , while it was the highest of 70.7 % for MDRD2-IDMS in stage 4 .
	manualset3
166636	7	412651	7	NULL	NULL	0	NULL	 stage 4	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Accuracy was the best at 75.1 % for Virga in stage 3 , while it was the highest of 70.7 % for MDRD2-IDMS in stage 4 .
	manualset3
166637	1	412652	7	NULL	NULL	0	NULL	structures 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structures of the transition states for a variety of enzyme-catalyzed ribosyl group transfer reactions , determined by computational evaluation of multiple tritium and heavy atom kinetic isotope effects on these enzymatic reactions , have been found to show a considerable variation in the extent of bond cleavage at the ribosyl anomeric carbon .
	manualset3
166638	2	412652	7	NULL	NULL	0	NULL	transition states 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The structures of the transition states for a variety of enzyme-catalyzed ribosyl group transfer reactions , determined by computational evaluation of multiple tritium and heavy atom kinetic isotope effects on these enzymatic reactions , have been found to show a considerable variation in the extent of bond cleavage at the ribosyl anomeric carbon .
	manualset3
166639	3	412652	7	NULL	NULL	0	NULL	enzyme-catalyzed ribosyl group transfer reactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The structures of the transition states for a variety of enzyme-catalyzed ribosyl group transfer reactions , determined by computational evaluation of multiple tritium and heavy atom kinetic isotope effects on these enzymatic reactions , have been found to show a considerable variation in the extent of bond cleavage at the ribosyl anomeric carbon .
	manualset3
166640	4	412652	7	NULL	NULL	0	NULL	computational evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structures of the transition states for a variety of enzyme-catalyzed ribosyl group transfer reactions , determined by computational evaluation of multiple tritium and heavy atom kinetic isotope effects on these enzymatic reactions , have been found to show a considerable variation in the extent of bond cleavage at the ribosyl anomeric carbon .
	manualset3
166641	5	412652	7	NULL	NULL	NULL	NULL	multiple tritium	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The structures of the transition states for a variety of enzyme-catalyzed ribosyl group transfer reactions , determined by computational evaluation of multiple tritium and heavy atom kinetic isotope effects on these enzymatic reactions , have been found to show a considerable variation in the extent of bond cleavage at the ribosyl anomeric carbon .
	manualset3
166642	6	412652	7	NULL	NULL	0	NULL	heavy atom kinetic isotope effects 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The structures of the transition states for a variety of enzyme-catalyzed ribosyl group transfer reactions , determined by computational evaluation of multiple tritium and heavy atom kinetic isotope effects on these enzymatic reactions , have been found to show a considerable variation in the extent of bond cleavage at the ribosyl anomeric carbon .
	manualset3
166643	7	412652	7	NULL	NULL	0	NULL	enzymatic reactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The structures of the transition states for a variety of enzyme-catalyzed ribosyl group transfer reactions , determined by computational evaluation of multiple tritium and heavy atom kinetic isotope effects on these enzymatic reactions , have been found to show a considerable variation in the extent of bond cleavage at the ribosyl anomeric carbon .
	manualset3
166644	8	412652	7	NULL	NULL	0	NULL	 variation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The structures of the transition states for a variety of enzyme-catalyzed ribosyl group transfer reactions , determined by computational evaluation of multiple tritium and heavy atom kinetic isotope effects on these enzymatic reactions , have been found to show a considerable variation in the extent of bond cleavage at the ribosyl anomeric carbon .
	manualset3
166645	9	412652	7	NULL	NULL	0	NULL	extent	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structures of the transition states for a variety of enzyme-catalyzed ribosyl group transfer reactions , determined by computational evaluation of multiple tritium and heavy atom kinetic isotope effects on these enzymatic reactions , have been found to show a considerable variation in the extent of bond cleavage at the ribosyl anomeric carbon .
	manualset3
166646	10	412652	7	NULL	NULL	0	NULL	bond cleavage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The structures of the transition states for a variety of enzyme-catalyzed ribosyl group transfer reactions , determined by computational evaluation of multiple tritium and heavy atom kinetic isotope effects on these enzymatic reactions , have been found to show a considerable variation in the extent of bond cleavage at the ribosyl anomeric carbon .
	manualset3
166647	11	412652	7	NULL	NULL	0	NULL	ribosyl anomeric carbon	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The structures of the transition states for a variety of enzyme-catalyzed ribosyl group transfer reactions , determined by computational evaluation of multiple tritium and heavy atom kinetic isotope effects on these enzymatic reactions , have been found to show a considerable variation in the extent of bond cleavage at the ribosyl anomeric carbon .
	manualset3
166648	1	412653	7	NULL	NULL	0	NULL	 studied drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The studied drug ( 0.5-5 mg/kg ) inhibited the spontaneous locomotor activity in mice .
	manualset3
166649	2	412653	7	NULL	NULL	0	NULL	0.5-5 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The studied drug ( 0.5-5 mg/kg ) inhibited the spontaneous locomotor activity in mice .
	manualset3
166650	3	412653	7	NULL	NULL	0	NULL	spontaneous locomotor activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The studied drug ( 0.5-5 mg/kg ) inhibited the spontaneous locomotor activity in mice .
	manualset3
166651	4	412653	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The studied drug ( 0.5-5 mg/kg ) inhibited the spontaneous locomotor activity in mice .
	manualset3
166652	1	412654	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The studies focused on the influence of various parameters ( e.g. , pH , kind of buffer , capillary wall ) on the electroosmotic flow ( EOF ) .
	manualset3
166653	2	412654	7	NULL	NULL	0	NULL	influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The studies focused on the influence of various parameters ( e.g. , pH , kind of buffer , capillary wall ) on the electroosmotic flow ( EOF ) .
	manualset3
166654	3	412654	7	NULL	NULL	0	NULL	parameters	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The studies focused on the influence of various parameters ( e.g. , pH , kind of buffer , capillary wall ) on the electroosmotic flow ( EOF ) .
	manualset3
166655	4	412654	7	NULL	NULL	0	NULL	pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The studies focused on the influence of various parameters ( e.g. , pH , kind of buffer , capillary wall ) on the electroosmotic flow ( EOF ) .
	manualset3
166656	5	412654	7	NULL	NULL	0	NULL	buffer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The studies focused on the influence of various parameters ( e.g. , pH , kind of buffer , capillary wall ) on the electroosmotic flow ( EOF ) .
	manualset3
166657	6	412654	7	NULL	NULL	0	NULL	capillary wall	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The studies focused on the influence of various parameters ( e.g. , pH , kind of buffer , capillary wall ) on the electroosmotic flow ( EOF ) .
	manualset3
166658	7	412654	7	NULL	NULL	0	NULL	electroosmotic flow ( EOF )	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The studies focused on the influence of various parameters ( e.g. , pH , kind of buffer , capillary wall ) on the electroosmotic flow ( EOF ) .
	manualset3
166659	1	412655	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study added some additional insights to the following questions : What costs should be collected , what level of detail is required for that task , what patients should by analyzed , and what data sources should be used in further studies in RA .
	manualset3
166660	2	412655	7	NULL	NULL	0	NULL	questions	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The study added some additional insights to the following questions : What costs should be collected , what level of detail is required for that task , what patients should by analyzed , and what data sources should be used in further studies in RA .
	manualset3
166661	3	412655	7	NULL	NULL	0	NULL	costs	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study added some additional insights to the following questions : What costs should be collected , what level of detail is required for that task , what patients should by analyzed , and what data sources should be used in further studies in RA .
	manualset3
166662	4	412655	7	NULL	NULL	0	NULL	 task	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The study added some additional insights to the following questions : What costs should be collected , what level of detail is required for that task , what patients should by analyzed , and what data sources should be used in further studies in RA .
	manualset3
166663	5	412655	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The study added some additional insights to the following questions : What costs should be collected , what level of detail is required for that task , what patients should by analyzed , and what data sources should be used in further studies in RA .
	manualset3
166664	6	412655	7	NULL	NULL	0	NULL	data sources	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The study added some additional insights to the following questions : What costs should be collected , what level of detail is required for that task , what patients should by analyzed , and what data sources should be used in further studies in RA .
	manualset3
166665	7	412655	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study added some additional insights to the following questions : What costs should be collected , what level of detail is required for that task , what patients should by analyzed , and what data sources should be used in further studies in RA .
	manualset3
166666	8	412655	7	NULL	NULL	0	NULL	RA	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study added some additional insights to the following questions : What costs should be collected , what level of detail is required for that task , what patients should by analyzed , and what data sources should be used in further studies in RA .
	manualset3
167783	9	412655	7	NULL	NULL	NULL	NULL	level 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study added some additional insights to the following questions : What costs should be collected , what level of detail is required for that task , what patients should by analyzed , and what data sources should be used in further studies in RA .
	manualset3
167784	10	412655	7	NULL	NULL	0	NULL	detail	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The study added some additional insights to the following questions : What costs should be collected , what level of detail is required for that task , what patients should by analyzed , and what data sources should be used in further studies in RA .
	manualset3
169195	11	412655	7	NULL	NULL	0	NULL	insights	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The study added some additional insights to the following questions : What costs should be collected , what level of detail is required for that task , what patients should by analyzed , and what data sources should be used in further studies in RA .
	manualset3
166667	1	412656	7	NULL	NULL	0	NULL	Accurate diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Accurate diagnosis and selection of the appropriate intervention depends on recognition of pertinent clinical and radiographic features .
	manualset3
166668	2	412656	7	NULL	NULL	0	NULL	selection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Accurate diagnosis and selection of the appropriate intervention depends on recognition of pertinent clinical and radiographic features .
	manualset3
166669	3	412656	7	NULL	NULL	0	NULL	 intervention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Accurate diagnosis and selection of the appropriate intervention depends on recognition of pertinent clinical and radiographic features .
	manualset3
166670	4	412656	7	NULL	NULL	0	NULL	 recognition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Accurate diagnosis and selection of the appropriate intervention depends on recognition of pertinent clinical and radiographic features .
	manualset3
166671	5	412656	7	NULL	NULL	0	NULL	pertinent clinical feature	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Accurate diagnosis and selection of the appropriate intervention depends on recognition of pertinent clinical and radiographic features .
	manualset3
166672	6	412656	7	NULL	NULL	0	NULL	radiographic features	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Accurate diagnosis and selection of the appropriate intervention depends on recognition of pertinent clinical and radiographic features .
	manualset3
166673	1	412657	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study aimed at investigation of the rate of periodontal pathologies in juvenile adolescents , the analysis of the severity of the disease and detection of the correlation between the periodontal tissue pathology and hormonal status of pre-and pubertal periods .
	manualset3
166674	2	412657	7	NULL	NULL	0	NULL	 investigation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study aimed at investigation of the rate of periodontal pathologies in juvenile adolescents , the analysis of the severity of the disease and detection of the correlation between the periodontal tissue pathology and hormonal status of pre-and pubertal periods .
	manualset3
166675	3	412657	7	NULL	NULL	0	NULL	 rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study aimed at investigation of the rate of periodontal pathologies in juvenile adolescents , the analysis of the severity of the disease and detection of the correlation between the periodontal tissue pathology and hormonal status of pre-and pubertal periods .
	manualset3
166676	4	412657	7	NULL	NULL	0	NULL	periodontal pathologies	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The study aimed at investigation of the rate of periodontal pathologies in juvenile adolescents , the analysis of the severity of the disease and detection of the correlation between the periodontal tissue pathology and hormonal status of pre-and pubertal periods .
	manualset3
166677	5	412657	7	NULL	NULL	0	NULL	juvenile adolescents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The study aimed at investigation of the rate of periodontal pathologies in juvenile adolescents , the analysis of the severity of the disease and detection of the correlation between the periodontal tissue pathology and hormonal status of pre-and pubertal periods .
	manualset3
166678	6	412657	7	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study aimed at investigation of the rate of periodontal pathologies in juvenile adolescents , the analysis of the severity of the disease and detection of the correlation between the periodontal tissue pathology and hormonal status of pre-and pubertal periods .
	manualset3
166679	7	412657	7	NULL	NULL	0	NULL	severity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study aimed at investigation of the rate of periodontal pathologies in juvenile adolescents , the analysis of the severity of the disease and detection of the correlation between the periodontal tissue pathology and hormonal status of pre-and pubertal periods .
	manualset3
166680	8	412657	7	NULL	NULL	0	NULL	 disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The study aimed at investigation of the rate of periodontal pathologies in juvenile adolescents , the analysis of the severity of the disease and detection of the correlation between the periodontal tissue pathology and hormonal status of pre-and pubertal periods .
	manualset3
166681	9	412657	7	NULL	NULL	0	NULL	detection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study aimed at investigation of the rate of periodontal pathologies in juvenile adolescents , the analysis of the severity of the disease and detection of the correlation between the periodontal tissue pathology and hormonal status of pre-and pubertal periods .
	manualset3
166682	10	412657	7	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The study aimed at investigation of the rate of periodontal pathologies in juvenile adolescents , the analysis of the severity of the disease and detection of the correlation between the periodontal tissue pathology and hormonal status of pre-and pubertal periods .
	manualset3
166683	11	412657	7	NULL	NULL	0	NULL	periodontal tissue pathology	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The study aimed at investigation of the rate of periodontal pathologies in juvenile adolescents , the analysis of the severity of the disease and detection of the correlation between the periodontal tissue pathology and hormonal status of pre-and pubertal periods .
	manualset3
166684	12	412657	7	NULL	NULL	0	NULL	hormonal status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study aimed at investigation of the rate of periodontal pathologies in juvenile adolescents , the analysis of the severity of the disease and detection of the correlation between the periodontal tissue pathology and hormonal status of pre-and pubertal periods .
	manualset3
166685	13	412657	7	NULL	NULL	0	NULL	pre-and pubertal periods	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study aimed at investigation of the rate of periodontal pathologies in juvenile adolescents , the analysis of the severity of the disease and detection of the correlation between the periodontal tissue pathology and hormonal status of pre-and pubertal periods .
	manualset3
166686	1	412658	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study assessed the long-term outcome of patients undergoing radiofrequency ablation of the right bundle for bundle branch reentrant ventricular tachycardia .
	manualset3
166687	2	412658	7	NULL	NULL	0	NULL	long-term outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study assessed the long-term outcome of patients undergoing radiofrequency ablation of the right bundle for bundle branch reentrant ventricular tachycardia .
	manualset3
166688	3	412658	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The study assessed the long-term outcome of patients undergoing radiofrequency ablation of the right bundle for bundle branch reentrant ventricular tachycardia .
	manualset3
166689	4	412658	7	NULL	NULL	0	NULL	radiofrequency ablation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The study assessed the long-term outcome of patients undergoing radiofrequency ablation of the right bundle for bundle branch reentrant ventricular tachycardia .
	manualset3
166690	5	412658	7	NULL	NULL	0	NULL	right bundle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The study assessed the long-term outcome of patients undergoing radiofrequency ablation of the right bundle for bundle branch reentrant ventricular tachycardia .
	manualset3
166691	6	412658	7	NULL	NULL	NULL	NULL	bundle branch reentrant ventricular tachycardia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study assessed the long-term outcome of patients undergoing radiofrequency ablation of the right bundle for bundle branch reentrant ventricular tachycardia .
	manualset3
166693	1	412659	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study compared immediate versus deferred treatment with the antiviral drug for CMV retinitis in people with AIDS .
	manualset3
166694	2	412659	7	NULL	NULL	0	NULL	 immediate treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The study compared immediate versus deferred treatment with the antiviral drug for CMV retinitis in people with AIDS .
	manualset3
166695	3	412659	7	NULL	NULL	0	NULL	deferred treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The study compared immediate versus deferred treatment with the antiviral drug for CMV retinitis in people with AIDS .
	manualset3
166696	4	412659	7	NULL	NULL	0	NULL	antiviral drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The study compared immediate versus deferred treatment with the antiviral drug for CMV retinitis in people with AIDS .
	manualset3
166697	5	412659	7	NULL	NULL	0	NULL	CMV retinitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study compared immediate versus deferred treatment with the antiviral drug for CMV retinitis in people with AIDS .
	manualset3
166698	6	412659	7	NULL	NULL	0	NULL	people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The study compared immediate versus deferred treatment with the antiviral drug for CMV retinitis in people with AIDS .
	manualset3
166699	7	412659	7	NULL	NULL	0	NULL	AIDS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study compared immediate versus deferred treatment with the antiviral drug for CMV retinitis in people with AIDS .
	manualset3
166700	1	412660	7	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study confirms the limitations of X-ray pelvimetry measurements and proposes that antenatal estimation of fetal size may be of benefit in determining the likelihood of success in a trial labor .
	manualset3
166701	2	412660	7	NULL	NULL	0	NULL	 limitations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study confirms the limitations of X-ray pelvimetry measurements and proposes that antenatal estimation of fetal size may be of benefit in determining the likelihood of success in a trial labor .
	manualset3
166702	3	412660	7	NULL	NULL	0	NULL	X-ray pelvimetry measurements	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study confirms the limitations of X-ray pelvimetry measurements and proposes that antenatal estimation of fetal size may be of benefit in determining the likelihood of success in a trial labor .
	manualset3
166703	4	412660	7	NULL	NULL	0	NULL	antenatal estimation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study confirms the limitations of X-ray pelvimetry measurements and proposes that antenatal estimation of fetal size may be of benefit in determining the likelihood of success in a trial labor .
	manualset3
166704	5	412660	7	NULL	NULL	0	NULL	fetal size	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study confirms the limitations of X-ray pelvimetry measurements and proposes that antenatal estimation of fetal size may be of benefit in determining the likelihood of success in a trial labor .
	manualset3
166705	6	412660	7	NULL	NULL	0	NULL	success	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study confirms the limitations of X-ray pelvimetry measurements and proposes that antenatal estimation of fetal size may be of benefit in determining the likelihood of success in a trial labor .
	manualset3
166706	7	412660	7	NULL	NULL	0	NULL	trial labor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study confirms the limitations of X-ray pelvimetry measurements and proposes that antenatal estimation of fetal size may be of benefit in determining the likelihood of success in a trial labor .
	manualset3
173648	8	412660	7	NULL	NULL	0	NULL	 likelihood 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study confirms the limitations of X-ray pelvimetry measurements and proposes that antenatal estimation of fetal size may be of benefit in determining the likelihood of success in a trial labor .
	manualset3
166707	1	412661	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study consisted of the determination of dust size distribution and of the size distribution of radionuclides associated with particulate matter in the size range less than 0.1 to 26 microns .
	manualset3
166708	2	412661	7	NULL	NULL	0	NULL	determination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study consisted of the determination of dust size distribution and of the size distribution of radionuclides associated with particulate matter in the size range less than 0.1 to 26 microns .
	manualset3
166709	3	412661	7	NULL	NULL	NULL	NULL	dust size distribution	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study consisted of the determination of dust size distribution and of the size distribution of radionuclides associated with particulate matter in the size range less than 0.1 to 26 microns .
	manualset3
166710	4	412661	7	NULL	NULL	NULL	NULL	size distribution 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study consisted of the determination of dust size distribution and of the size distribution of radionuclides associated with particulate matter in the size range less than 0.1 to 26 microns .
	manualset3
166711	5	412661	7	NULL	NULL	0	NULL	radionuclides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The study consisted of the determination of dust size distribution and of the size distribution of radionuclides associated with particulate matter in the size range less than 0.1 to 26 microns .
	manualset3
166712	6	412661	7	NULL	NULL	0	NULL	particulate matter	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The study consisted of the determination of dust size distribution and of the size distribution of radionuclides associated with particulate matter in the size range less than 0.1 to 26 microns .
	manualset3
166713	7	412661	7	NULL	NULL	0	NULL	size range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study consisted of the determination of dust size distribution and of the size distribution of radionuclides associated with particulate matter in the size range less than 0.1 to 26 microns .
	manualset3
166714	8	412661	7	NULL	NULL	0	NULL	0.1 to 26 microns	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The study consisted of the determination of dust size distribution and of the size distribution of radionuclides associated with particulate matter in the size range less than 0.1 to 26 microns .
	manualset3
166715	1	412662	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study described in this paper was primarily conducted to identify the cell types involved in the formation , progression and regression of metaplastic changes in the respiratory tract epithelium of hamsters after intratracheal intubations with benzo ( a ) pyrene .
	manualset3
166716	2	412662	7	NULL	NULL	0	NULL	paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The study described in this paper was primarily conducted to identify the cell types involved in the formation , progression and regression of metaplastic changes in the respiratory tract epithelium of hamsters after intratracheal intubations with benzo ( a ) pyrene .
	manualset3
166717	3	412662	7	NULL	NULL	0	NULL	cell types	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The study described in this paper was primarily conducted to identify the cell types involved in the formation , progression and regression of metaplastic changes in the respiratory tract epithelium of hamsters after intratracheal intubations with benzo ( a ) pyrene .
	manualset3
166718	4	412662	7	NULL	NULL	0	NULL	formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The study described in this paper was primarily conducted to identify the cell types involved in the formation , progression and regression of metaplastic changes in the respiratory tract epithelium of hamsters after intratracheal intubations with benzo ( a ) pyrene .
	manualset3
166719	5	412662	7	NULL	NULL	0	NULL	progression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The study described in this paper was primarily conducted to identify the cell types involved in the formation , progression and regression of metaplastic changes in the respiratory tract epithelium of hamsters after intratracheal intubations with benzo ( a ) pyrene .
	manualset3
166720	6	412662	7	NULL	NULL	0	NULL	regression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The study described in this paper was primarily conducted to identify the cell types involved in the formation , progression and regression of metaplastic changes in the respiratory tract epithelium of hamsters after intratracheal intubations with benzo ( a ) pyrene .
	manualset3
166721	7	412662	7	NULL	NULL	0	NULL	metaplastic changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study described in this paper was primarily conducted to identify the cell types involved in the formation , progression and regression of metaplastic changes in the respiratory tract epithelium of hamsters after intratracheal intubations with benzo ( a ) pyrene .
	manualset3
166722	8	412662	7	NULL	NULL	0	NULL	respiratory tract epithelium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The study described in this paper was primarily conducted to identify the cell types involved in the formation , progression and regression of metaplastic changes in the respiratory tract epithelium of hamsters after intratracheal intubations with benzo ( a ) pyrene .
	manualset3
166723	9	412662	7	NULL	NULL	0	NULL	hamsters	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The study described in this paper was primarily conducted to identify the cell types involved in the formation , progression and regression of metaplastic changes in the respiratory tract epithelium of hamsters after intratracheal intubations with benzo ( a ) pyrene .
	manualset3
166724	10	412662	7	NULL	NULL	0	NULL	intratracheal intubations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The study described in this paper was primarily conducted to identify the cell types involved in the formation , progression and regression of metaplastic changes in the respiratory tract epithelium of hamsters after intratracheal intubations with benzo ( a ) pyrene .
	manualset3
166725	11	412662	7	NULL	NULL	0	NULL	 benzo ( a ) pyrene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The study described in this paper was primarily conducted to identify the cell types involved in the formation , progression and regression of metaplastic changes in the respiratory tract epithelium of hamsters after intratracheal intubations with benzo ( a ) pyrene .
	manualset3
166726	1	412663	7	NULL	NULL	0	NULL	study documents	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The study documents that caring for older people is about creating small everyday circumstances in which patient dignity can flourish .
	manualset3
166727	2	412663	7	NULL	NULL	0	NULL	older people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The study documents that caring for older people is about creating small everyday circumstances in which patient dignity can flourish .
	manualset3
166728	3	412663	7	NULL	NULL	NULL	NULL	everyday circumstances 	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study documents that caring for older people is about creating small everyday circumstances in which patient dignity can flourish .
	manualset3
166729	4	412663	7	NULL	NULL	0	NULL	patient dignity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study documents that caring for older people is about creating small everyday circumstances in which patient dignity can flourish .
	manualset3
166730	1	412664	7	NULL	NULL	0	NULL	Accurate estimation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Accurate estimation of the human head conductivity is important for the diagnosis and therapy of brain diseases .
	manualset3
166731	2	412664	7	NULL	NULL	0	NULL	human head conductivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Accurate estimation of the human head conductivity is important for the diagnosis and therapy of brain diseases .
	manualset3
166732	3	412664	7	NULL	NULL	0	NULL	diagnosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Accurate estimation of the human head conductivity is important for the diagnosis and therapy of brain diseases .
	manualset3
166733	4	412664	7	NULL	NULL	0	NULL	 therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Accurate estimation of the human head conductivity is important for the diagnosis and therapy of brain diseases .
	manualset3
166734	5	412664	7	NULL	NULL	0	NULL	brain diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Accurate estimation of the human head conductivity is important for the diagnosis and therapy of brain diseases .
	manualset3
166735	1	412665	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study enrolled 300 women submitted to a clinical protocol using cytological examination alone , digital cervicography without image magnification ( Evaluation 1 ) , and digital cervicography plus additional image magnification and considering the positive criteria ( Evaluation 2 ) .
	manualset3
166736	2	412665	7	NULL	NULL	0	NULL	300 women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The study enrolled 300 women submitted to a clinical protocol using cytological examination alone , digital cervicography without image magnification ( Evaluation 1 ) , and digital cervicography plus additional image magnification and considering the positive criteria ( Evaluation 2 ) .
	manualset3
166737	3	412665	7	NULL	NULL	0	NULL	clinical protocol	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The study enrolled 300 women submitted to a clinical protocol using cytological examination alone , digital cervicography without image magnification ( Evaluation 1 ) , and digital cervicography plus additional image magnification and considering the positive criteria ( Evaluation 2 ) .
	manualset3
166738	4	412665	7	NULL	NULL	0	NULL	cytological examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The study enrolled 300 women submitted to a clinical protocol using cytological examination alone , digital cervicography without image magnification ( Evaluation 1 ) , and digital cervicography plus additional image magnification and considering the positive criteria ( Evaluation 2 ) .
	manualset3
166739	5	412665	7	NULL	NULL	NULL	NULL	digital cervicography without image magnification ( Evaluation 1 )	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study enrolled 300 women submitted to a clinical protocol using cytological examination alone , digital cervicography without image magnification ( Evaluation 1 ) , and digital cervicography plus additional image magnification and considering the positive criteria ( Evaluation 2 ) .
	manualset3
166741	6	412665	7	NULL	NULL	NULL	NULL	digital cervicography plus additional image magnification	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study enrolled 300 women submitted to a clinical protocol using cytological examination alone , digital cervicography without image magnification ( Evaluation 1 ) , and digital cervicography plus additional image magnification and considering the positive criteria ( Evaluation 2 ) .
	manualset3
166743	7	412665	7	NULL	NULL	NULL	NULL	positive criteria ( Evaluation 2 )	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study enrolled 300 women submitted to a clinical protocol using cytological examination alone , digital cervicography without image magnification ( Evaluation 1 ) , and digital cervicography plus additional image magnification and considering the positive criteria ( Evaluation 2 ) .
	manualset3
166744	1	412666	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study explored the relations of visual perceptual deficits and motor impairments in 60 children with Developmental Coordination Disorder ( 120.8 + / - 4.0 mo. ) and 60 controls ( 121.0 + / - 5.3 mo. ) , who were matched by sex ( 29 boys and 31 girls ) and age .
	manualset3
166745	2	412666	7	NULL	NULL	0	NULL	 relations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The study explored the relations of visual perceptual deficits and motor impairments in 60 children with Developmental Coordination Disorder ( 120.8 + / - 4.0 mo. ) and 60 controls ( 121.0 + / - 5.3 mo. ) , who were matched by sex ( 29 boys and 31 girls ) and age .
	manualset3
166746	3	412666	7	NULL	NULL	0	NULL	visual perceptual deficits 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study explored the relations of visual perceptual deficits and motor impairments in 60 children with Developmental Coordination Disorder ( 120.8 + / - 4.0 mo. ) and 60 controls ( 121.0 + / - 5.3 mo. ) , who were matched by sex ( 29 boys and 31 girls ) and age .
	manualset3
166747	4	412666	7	NULL	NULL	0	NULL	motor impairments 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study explored the relations of visual perceptual deficits and motor impairments in 60 children with Developmental Coordination Disorder ( 120.8 + / - 4.0 mo. ) and 60 controls ( 121.0 + / - 5.3 mo. ) , who were matched by sex ( 29 boys and 31 girls ) and age .
	manualset3
166748	5	412666	7	NULL	NULL	0	NULL	60 children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The study explored the relations of visual perceptual deficits and motor impairments in 60 children with Developmental Coordination Disorder ( 120.8 + / - 4.0 mo. ) and 60 controls ( 121.0 + / - 5.3 mo. ) , who were matched by sex ( 29 boys and 31 girls ) and age .
	manualset3
166749	6	412666	7	NULL	NULL	NULL	NULL	Developmental Coordination Disorder	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study explored the relations of visual perceptual deficits and motor impairments in 60 children with Developmental Coordination Disorder ( 120.8 + / - 4.0 mo. ) and 60 controls ( 121.0 + / - 5.3 mo. ) , who were matched by sex ( 29 boys and 31 girls ) and age .
	manualset3
166750	7	412666	7	NULL	NULL	0	NULL	120.8 + / - 4.0 mo	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The study explored the relations of visual perceptual deficits and motor impairments in 60 children with Developmental Coordination Disorder ( 120.8 + / - 4.0 mo. ) and 60 controls ( 121.0 + / - 5.3 mo. ) , who were matched by sex ( 29 boys and 31 girls ) and age .
	manualset3
166751	8	412666	7	NULL	NULL	0	NULL	60 controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The study explored the relations of visual perceptual deficits and motor impairments in 60 children with Developmental Coordination Disorder ( 120.8 + / - 4.0 mo. ) and 60 controls ( 121.0 + / - 5.3 mo. ) , who were matched by sex ( 29 boys and 31 girls ) and age .
	manualset3
166752	9	412666	7	NULL	NULL	0	NULL	121.0 + / - 5.3 mo.	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The study explored the relations of visual perceptual deficits and motor impairments in 60 children with Developmental Coordination Disorder ( 120.8 + / - 4.0 mo. ) and 60 controls ( 121.0 + / - 5.3 mo. ) , who were matched by sex ( 29 boys and 31 girls ) and age .
	manualset3
166753	10	412666	7	NULL	NULL	0	NULL	sex	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study explored the relations of visual perceptual deficits and motor impairments in 60 children with Developmental Coordination Disorder ( 120.8 + / - 4.0 mo. ) and 60 controls ( 121.0 + / - 5.3 mo. ) , who were matched by sex ( 29 boys and 31 girls ) and age .
	manualset3
166754	11	412666	7	NULL	NULL	0	NULL	29 boys	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The study explored the relations of visual perceptual deficits and motor impairments in 60 children with Developmental Coordination Disorder ( 120.8 + / - 4.0 mo. ) and 60 controls ( 121.0 + / - 5.3 mo. ) , who were matched by sex ( 29 boys and 31 girls ) and age .
	manualset3
166755	12	412666	7	NULL	NULL	0	NULL	31 girls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The study explored the relations of visual perceptual deficits and motor impairments in 60 children with Developmental Coordination Disorder ( 120.8 + / - 4.0 mo. ) and 60 controls ( 121.0 + / - 5.3 mo. ) , who were matched by sex ( 29 boys and 31 girls ) and age .
	manualset3
166756	13	412666	7	NULL	NULL	NULL	NULL	age	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study explored the relations of visual perceptual deficits and motor impairments in 60 children with Developmental Coordination Disorder ( 120.8 + / - 4.0 mo. ) and 60 controls ( 121.0 + / - 5.3 mo. ) , who were matched by sex ( 29 boys and 31 girls ) and age .
	manualset3
166757	1	412667	7	NULL	NULL	NULL	NULL	 study findings	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study findings highlight the need for a research focus on the roles of mental health and other registered nurses who work with people receiving OST in specialist service and primary care settings , and endorse a partnership approach to future research in this area .
	manualset3
166758	2	412667	7	NULL	NULL	NULL	NULL	research focus	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study findings highlight the need for a research focus on the roles of mental health and other registered nurses who work with people receiving OST in specialist service and primary care settings , and endorse a partnership approach to future research in this area .
	manualset3
166759	3	412667	7	NULL	NULL	0	NULL	 roles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The study findings highlight the need for a research focus on the roles of mental health and other registered nurses who work with people receiving OST in specialist service and primary care settings , and endorse a partnership approach to future research in this area .
	manualset3
166760	4	412667	7	NULL	NULL	NULL	NULL	mental health	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study findings highlight the need for a research focus on the roles of mental health and other registered nurses who work with people receiving OST in specialist service and primary care settings , and endorse a partnership approach to future research in this area .
	manualset3
166761	5	412667	7	NULL	NULL	0	NULL	registered nurses	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The study findings highlight the need for a research focus on the roles of mental health and other registered nurses who work with people receiving OST in specialist service and primary care settings , and endorse a partnership approach to future research in this area .
	manualset3
166762	6	412667	7	NULL	NULL	0	NULL	people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The study findings highlight the need for a research focus on the roles of mental health and other registered nurses who work with people receiving OST in specialist service and primary care settings , and endorse a partnership approach to future research in this area .
	manualset3
166763	7	412667	7	NULL	NULL	0	NULL	OST	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study findings highlight the need for a research focus on the roles of mental health and other registered nurses who work with people receiving OST in specialist service and primary care settings , and endorse a partnership approach to future research in this area .
	manualset3
166764	8	412667	7	NULL	NULL	0	NULL	specialist service	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The study findings highlight the need for a research focus on the roles of mental health and other registered nurses who work with people receiving OST in specialist service and primary care settings , and endorse a partnership approach to future research in this area .
	manualset3
166765	9	412667	7	NULL	NULL	0	NULL	primary care settings	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The study findings highlight the need for a research focus on the roles of mental health and other registered nurses who work with people receiving OST in specialist service and primary care settings , and endorse a partnership approach to future research in this area .
	manualset3
166766	10	412667	7	NULL	NULL	0	NULL	partnership approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study findings highlight the need for a research focus on the roles of mental health and other registered nurses who work with people receiving OST in specialist service and primary care settings , and endorse a partnership approach to future research in this area .
	manualset3
166767	11	412667	7	NULL	NULL	0	NULL	future research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study findings highlight the need for a research focus on the roles of mental health and other registered nurses who work with people receiving OST in specialist service and primary care settings , and endorse a partnership approach to future research in this area .
	manualset3
166768	12	412667	7	NULL	NULL	0	NULL	area	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study findings highlight the need for a research focus on the roles of mental health and other registered nurses who work with people receiving OST in specialist service and primary care settings , and endorse a partnership approach to future research in this area .
	manualset3
169196	13	412667	7	NULL	NULL	0	NULL	need	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study findings highlight the need for a research focus on the roles of mental health and other registered nurses who work with people receiving OST in specialist service and primary care settings , and endorse a partnership approach to future research in this area .
	manualset3
166769	1	412668	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study identified the need for nurses and other health care providers to be aware of the influence these ethical principles have on decision making and the importance of autonomy to the parents of well children .
	manualset3
166770	2	412668	7	NULL	NULL	0	NULL	nurses	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The study identified the need for nurses and other health care providers to be aware of the influence these ethical principles have on decision making and the importance of autonomy to the parents of well children .
	manualset3
166771	3	412668	7	NULL	NULL	0	NULL	health care providers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The study identified the need for nurses and other health care providers to be aware of the influence these ethical principles have on decision making and the importance of autonomy to the parents of well children .
	manualset3
166772	4	412668	7	NULL	NULL	NULL	NULL	ethical principles	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study identified the need for nurses and other health care providers to be aware of the influence these ethical principles have on decision making and the importance of autonomy to the parents of well children .
	manualset3
166773	5	412668	7	NULL	NULL	0	NULL	decision making	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The study identified the need for nurses and other health care providers to be aware of the influence these ethical principles have on decision making and the importance of autonomy to the parents of well children .
	manualset3
166774	6	412668	7	NULL	NULL	NULL	NULL	importance of autonomy	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study identified the need for nurses and other health care providers to be aware of the influence these ethical principles have on decision making and the importance of autonomy to the parents of well children .
	manualset3
166775	7	412668	7	NULL	NULL	0	NULL	parents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The study identified the need for nurses and other health care providers to be aware of the influence these ethical principles have on decision making and the importance of autonomy to the parents of well children .
	manualset3
166776	8	412668	7	NULL	NULL	0	NULL	well children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The study identified the need for nurses and other health care providers to be aware of the influence these ethical principles have on decision making and the importance of autonomy to the parents of well children .
	manualset3
169197	9	412668	7	NULL	NULL	0	NULL	need	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study identified the need for nurses and other health care providers to be aware of the influence these ethical principles have on decision making and the importance of autonomy to the parents of well children .
	manualset3
169198	10	412668	7	NULL	NULL	0	NULL	influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The study identified the need for nurses and other health care providers to be aware of the influence these ethical principles have on decision making and the importance of autonomy to the parents of well children .
	manualset3
166777	1	412669	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study included 46 samples from patients with non-metastatic squamous cell carcinoma of the larynx without any previous oncological treatments .
	manualset3
166778	2	412669	7	NULL	NULL	NULL	NULL	 46 samples	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study included 46 samples from patients with non-metastatic squamous cell carcinoma of the larynx without any previous oncological treatments .
	manualset3
166779	3	412669	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The study included 46 samples from patients with non-metastatic squamous cell carcinoma of the larynx without any previous oncological treatments .
	manualset3
166780	4	412669	7	NULL	NULL	NULL	NULL	non-metastatic squamous cell carcinoma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study included 46 samples from patients with non-metastatic squamous cell carcinoma of the larynx without any previous oncological treatments .
	manualset3
166781	6	412669	7	NULL	NULL	NULL	NULL	oncological treatments	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study included 46 samples from patients with non-metastatic squamous cell carcinoma of the larynx without any previous oncological treatments .
	manualset3
167786	5	412669	7	NULL	NULL	NULL	NULL	 larynx	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study included 46 samples from patients with non-metastatic squamous cell carcinoma of the larynx without any previous oncological treatments .
	manualset3
166782	1	412670	7	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study indicates that ( 18 ) F-FLT/microPET is a useful imaging modality for early detection of chemotherapy in the colorectal mouse model .
	manualset3
166783	2	412670	7	NULL	NULL	0	NULL	 F-FLT/microPET 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The study indicates that ( 18 ) F-FLT/microPET is a useful imaging modality for early detection of chemotherapy in the colorectal mouse model .
	manualset3
166784	3	412670	7	NULL	NULL	0	NULL	imaging modality	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The study indicates that ( 18 ) F-FLT/microPET is a useful imaging modality for early detection of chemotherapy in the colorectal mouse model .
	manualset3
166785	4	412670	7	NULL	NULL	0	NULL	early detection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study indicates that ( 18 ) F-FLT/microPET is a useful imaging modality for early detection of chemotherapy in the colorectal mouse model .
	manualset3
166786	5	412670	7	NULL	NULL	0	NULL	chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The study indicates that ( 18 ) F-FLT/microPET is a useful imaging modality for early detection of chemotherapy in the colorectal mouse model .
	manualset3
166787	6	412670	7	NULL	NULL	0	NULL	colorectal mouse model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The study indicates that ( 18 ) F-FLT/microPET is a useful imaging modality for early detection of chemotherapy in the colorectal mouse model .
	manualset3
166788	1	412671	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study indicates that 1 ) the parent-offspring and sibling correlation coefficients conformed with the theoretical correlations expected assuming polygenic inheritance ; 2 ) the husband-wife correlations indicate a high degree of assortative mating for skin color , but despite this effect the parent-offspring and sibling correlation coefficients are lower that the values expected under the influence of autosomal genes ; 3 ) estimates of heritability and components of phenotypic expression indicate that about 55 % of the total variability in skin reflectance could be attributed to the influence of additive genetic factors ; and 4 ) there is no evidence of X-linkage in the inheritance of skin color .
	manualset3
166789	2	412671	7	NULL	NULL	0	NULL	parent-offspring	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The study indicates that 1 ) the parent-offspring and sibling correlation coefficients conformed with the theoretical correlations expected assuming polygenic inheritance ; 2 ) the husband-wife correlations indicate a high degree of assortative mating for skin color , but despite this effect the parent-offspring and sibling correlation coefficients are lower that the values expected under the influence of autosomal genes ; 3 ) estimates of heritability and components of phenotypic expression indicate that about 55 % of the total variability in skin reflectance could be attributed to the influence of additive genetic factors ; and 4 ) there is no evidence of X-linkage in the inheritance of skin color .
	manualset3
166790	3	412671	7	NULL	NULL	NULL	NULL	sibling correlation coefficients	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study indicates that 1 ) the parent-offspring and sibling correlation coefficients conformed with the theoretical correlations expected assuming polygenic inheritance ; 2 ) the husband-wife correlations indicate a high degree of assortative mating for skin color , but despite this effect the parent-offspring and sibling correlation coefficients are lower that the values expected under the influence of autosomal genes ; 3 ) estimates of heritability and components of phenotypic expression indicate that about 55 % of the total variability in skin reflectance could be attributed to the influence of additive genetic factors ; and 4 ) there is no evidence of X-linkage in the inheritance of skin color .
	manualset3
166792	4	412671	7	NULL	NULL	NULL	NULL	theoretical correlations	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study indicates that 1 ) the parent-offspring and sibling correlation coefficients conformed with the theoretical correlations expected assuming polygenic inheritance ; 2 ) the husband-wife correlations indicate a high degree of assortative mating for skin color , but despite this effect the parent-offspring and sibling correlation coefficients are lower that the values expected under the influence of autosomal genes ; 3 ) estimates of heritability and components of phenotypic expression indicate that about 55 % of the total variability in skin reflectance could be attributed to the influence of additive genetic factors ; and 4 ) there is no evidence of X-linkage in the inheritance of skin color .
	manualset3
166793	5	412671	7	NULL	NULL	NULL	NULL	polygenic inheritance	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study indicates that 1 ) the parent-offspring and sibling correlation coefficients conformed with the theoretical correlations expected assuming polygenic inheritance ; 2 ) the husband-wife correlations indicate a high degree of assortative mating for skin color , but despite this effect the parent-offspring and sibling correlation coefficients are lower that the values expected under the influence of autosomal genes ; 3 ) estimates of heritability and components of phenotypic expression indicate that about 55 % of the total variability in skin reflectance could be attributed to the influence of additive genetic factors ; and 4 ) there is no evidence of X-linkage in the inheritance of skin color .
	manualset3
166794	6	412671	7	NULL	NULL	NULL	NULL	husband-wife correlations	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study indicates that 1 ) the parent-offspring and sibling correlation coefficients conformed with the theoretical correlations expected assuming polygenic inheritance ; 2 ) the husband-wife correlations indicate a high degree of assortative mating for skin color , but despite this effect the parent-offspring and sibling correlation coefficients are lower that the values expected under the influence of autosomal genes ; 3 ) estimates of heritability and components of phenotypic expression indicate that about 55 % of the total variability in skin reflectance could be attributed to the influence of additive genetic factors ; and 4 ) there is no evidence of X-linkage in the inheritance of skin color .
	manualset3
166796	8	412671	7	NULL	NULL	NULL	NULL	high degree 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study indicates that 1 ) the parent-offspring and sibling correlation coefficients conformed with the theoretical correlations expected assuming polygenic inheritance ; 2 ) the husband-wife correlations indicate a high degree of assortative mating for skin color , but despite this effect the parent-offspring and sibling correlation coefficients are lower that the values expected under the influence of autosomal genes ; 3 ) estimates of heritability and components of phenotypic expression indicate that about 55 % of the total variability in skin reflectance could be attributed to the influence of additive genetic factors ; and 4 ) there is no evidence of X-linkage in the inheritance of skin color .
	manualset3
166797	9	412671	7	NULL	NULL	NULL	NULL	assortative mating	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study indicates that 1 ) the parent-offspring and sibling correlation coefficients conformed with the theoretical correlations expected assuming polygenic inheritance ; 2 ) the husband-wife correlations indicate a high degree of assortative mating for skin color , but despite this effect the parent-offspring and sibling correlation coefficients are lower that the values expected under the influence of autosomal genes ; 3 ) estimates of heritability and components of phenotypic expression indicate that about 55 % of the total variability in skin reflectance could be attributed to the influence of additive genetic factors ; and 4 ) there is no evidence of X-linkage in the inheritance of skin color .
	manualset3
166798	10	412671	7	NULL	NULL	NULL	NULL	skin color	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study indicates that 1 ) the parent-offspring and sibling correlation coefficients conformed with the theoretical correlations expected assuming polygenic inheritance ; 2 ) the husband-wife correlations indicate a high degree of assortative mating for skin color , but despite this effect the parent-offspring and sibling correlation coefficients are lower that the values expected under the influence of autosomal genes ; 3 ) estimates of heritability and components of phenotypic expression indicate that about 55 % of the total variability in skin reflectance could be attributed to the influence of additive genetic factors ; and 4 ) there is no evidence of X-linkage in the inheritance of skin color .
	manualset3
166799	11	412671	7	NULL	NULL	0	NULL	parent-offspring 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The study indicates that 1 ) the parent-offspring and sibling correlation coefficients conformed with the theoretical correlations expected assuming polygenic inheritance ; 2 ) the husband-wife correlations indicate a high degree of assortative mating for skin color , but despite this effect the parent-offspring and sibling correlation coefficients are lower that the values expected under the influence of autosomal genes ; 3 ) estimates of heritability and components of phenotypic expression indicate that about 55 % of the total variability in skin reflectance could be attributed to the influence of additive genetic factors ; and 4 ) there is no evidence of X-linkage in the inheritance of skin color .
	manualset3
166800	12	412671	7	NULL	NULL	0	NULL	sibling correlation coefficients	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The study indicates that 1 ) the parent-offspring and sibling correlation coefficients conformed with the theoretical correlations expected assuming polygenic inheritance ; 2 ) the husband-wife correlations indicate a high degree of assortative mating for skin color , but despite this effect the parent-offspring and sibling correlation coefficients are lower that the values expected under the influence of autosomal genes ; 3 ) estimates of heritability and components of phenotypic expression indicate that about 55 % of the total variability in skin reflectance could be attributed to the influence of additive genetic factors ; and 4 ) there is no evidence of X-linkage in the inheritance of skin color .
	manualset3
166801	13	412671	7	NULL	NULL	0	NULL	values 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study indicates that 1 ) the parent-offspring and sibling correlation coefficients conformed with the theoretical correlations expected assuming polygenic inheritance ; 2 ) the husband-wife correlations indicate a high degree of assortative mating for skin color , but despite this effect the parent-offspring and sibling correlation coefficients are lower that the values expected under the influence of autosomal genes ; 3 ) estimates of heritability and components of phenotypic expression indicate that about 55 % of the total variability in skin reflectance could be attributed to the influence of additive genetic factors ; and 4 ) there is no evidence of X-linkage in the inheritance of skin color .
	manualset3
166802	14	412671	7	NULL	NULL	NULL	NULL	 influence	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study indicates that 1 ) the parent-offspring and sibling correlation coefficients conformed with the theoretical correlations expected assuming polygenic inheritance ; 2 ) the husband-wife correlations indicate a high degree of assortative mating for skin color , but despite this effect the parent-offspring and sibling correlation coefficients are lower that the values expected under the influence of autosomal genes ; 3 ) estimates of heritability and components of phenotypic expression indicate that about 55 % of the total variability in skin reflectance could be attributed to the influence of additive genetic factors ; and 4 ) there is no evidence of X-linkage in the inheritance of skin color .
	manualset3
166803	15	412671	7	NULL	NULL	0	NULL	autosomal genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The study indicates that 1 ) the parent-offspring and sibling correlation coefficients conformed with the theoretical correlations expected assuming polygenic inheritance ; 2 ) the husband-wife correlations indicate a high degree of assortative mating for skin color , but despite this effect the parent-offspring and sibling correlation coefficients are lower that the values expected under the influence of autosomal genes ; 3 ) estimates of heritability and components of phenotypic expression indicate that about 55 % of the total variability in skin reflectance could be attributed to the influence of additive genetic factors ; and 4 ) there is no evidence of X-linkage in the inheritance of skin color .
	manualset3
166804	16	412671	7	NULL	NULL	NULL	NULL	estimates of heritability	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study indicates that 1 ) the parent-offspring and sibling correlation coefficients conformed with the theoretical correlations expected assuming polygenic inheritance ; 2 ) the husband-wife correlations indicate a high degree of assortative mating for skin color , but despite this effect the parent-offspring and sibling correlation coefficients are lower that the values expected under the influence of autosomal genes ; 3 ) estimates of heritability and components of phenotypic expression indicate that about 55 % of the total variability in skin reflectance could be attributed to the influence of additive genetic factors ; and 4 ) there is no evidence of X-linkage in the inheritance of skin color .
	manualset3
166807	19	412671	7	NULL	NULL	0	NULL	phenotypic expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The study indicates that 1 ) the parent-offspring and sibling correlation coefficients conformed with the theoretical correlations expected assuming polygenic inheritance ; 2 ) the husband-wife correlations indicate a high degree of assortative mating for skin color , but despite this effect the parent-offspring and sibling correlation coefficients are lower that the values expected under the influence of autosomal genes ; 3 ) estimates of heritability and components of phenotypic expression indicate that about 55 % of the total variability in skin reflectance could be attributed to the influence of additive genetic factors ; and 4 ) there is no evidence of X-linkage in the inheritance of skin color .
	manualset3
166808	20	412671	7	NULL	NULL	0	NULL	55 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The study indicates that 1 ) the parent-offspring and sibling correlation coefficients conformed with the theoretical correlations expected assuming polygenic inheritance ; 2 ) the husband-wife correlations indicate a high degree of assortative mating for skin color , but despite this effect the parent-offspring and sibling correlation coefficients are lower that the values expected under the influence of autosomal genes ; 3 ) estimates of heritability and components of phenotypic expression indicate that about 55 % of the total variability in skin reflectance could be attributed to the influence of additive genetic factors ; and 4 ) there is no evidence of X-linkage in the inheritance of skin color .
	manualset3
166809	21	412671	7	NULL	NULL	0	NULL	 total variability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The study indicates that 1 ) the parent-offspring and sibling correlation coefficients conformed with the theoretical correlations expected assuming polygenic inheritance ; 2 ) the husband-wife correlations indicate a high degree of assortative mating for skin color , but despite this effect the parent-offspring and sibling correlation coefficients are lower that the values expected under the influence of autosomal genes ; 3 ) estimates of heritability and components of phenotypic expression indicate that about 55 % of the total variability in skin reflectance could be attributed to the influence of additive genetic factors ; and 4 ) there is no evidence of X-linkage in the inheritance of skin color .
	manualset3
166810	22	412671	7	NULL	NULL	0	NULL	skin reflectance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study indicates that 1 ) the parent-offspring and sibling correlation coefficients conformed with the theoretical correlations expected assuming polygenic inheritance ; 2 ) the husband-wife correlations indicate a high degree of assortative mating for skin color , but despite this effect the parent-offspring and sibling correlation coefficients are lower that the values expected under the influence of autosomal genes ; 3 ) estimates of heritability and components of phenotypic expression indicate that about 55 % of the total variability in skin reflectance could be attributed to the influence of additive genetic factors ; and 4 ) there is no evidence of X-linkage in the inheritance of skin color .
	manualset3
166811	23	412671	7	NULL	NULL	NULL	NULL	influence	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study indicates that 1 ) the parent-offspring and sibling correlation coefficients conformed with the theoretical correlations expected assuming polygenic inheritance ; 2 ) the husband-wife correlations indicate a high degree of assortative mating for skin color , but despite this effect the parent-offspring and sibling correlation coefficients are lower that the values expected under the influence of autosomal genes ; 3 ) estimates of heritability and components of phenotypic expression indicate that about 55 % of the total variability in skin reflectance could be attributed to the influence of additive genetic factors ; and 4 ) there is no evidence of X-linkage in the inheritance of skin color .
	manualset3
166812	24	412671	7	NULL	NULL	0	NULL	additive genetic factors	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The study indicates that 1 ) the parent-offspring and sibling correlation coefficients conformed with the theoretical correlations expected assuming polygenic inheritance ; 2 ) the husband-wife correlations indicate a high degree of assortative mating for skin color , but despite this effect the parent-offspring and sibling correlation coefficients are lower that the values expected under the influence of autosomal genes ; 3 ) estimates of heritability and components of phenotypic expression indicate that about 55 % of the total variability in skin reflectance could be attributed to the influence of additive genetic factors ; and 4 ) there is no evidence of X-linkage in the inheritance of skin color .
	manualset3
166813	25	412671	7	NULL	NULL	0	NULL	evidence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study indicates that 1 ) the parent-offspring and sibling correlation coefficients conformed with the theoretical correlations expected assuming polygenic inheritance ; 2 ) the husband-wife correlations indicate a high degree of assortative mating for skin color , but despite this effect the parent-offspring and sibling correlation coefficients are lower that the values expected under the influence of autosomal genes ; 3 ) estimates of heritability and components of phenotypic expression indicate that about 55 % of the total variability in skin reflectance could be attributed to the influence of additive genetic factors ; and 4 ) there is no evidence of X-linkage in the inheritance of skin color .
	manualset3
166814	26	412671	7	NULL	NULL	0	NULL	X-linkage 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The study indicates that 1 ) the parent-offspring and sibling correlation coefficients conformed with the theoretical correlations expected assuming polygenic inheritance ; 2 ) the husband-wife correlations indicate a high degree of assortative mating for skin color , but despite this effect the parent-offspring and sibling correlation coefficients are lower that the values expected under the influence of autosomal genes ; 3 ) estimates of heritability and components of phenotypic expression indicate that about 55 % of the total variability in skin reflectance could be attributed to the influence of additive genetic factors ; and 4 ) there is no evidence of X-linkage in the inheritance of skin color .
	manualset3
166815	27	412671	7	NULL	NULL	0	NULL	inheritance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The study indicates that 1 ) the parent-offspring and sibling correlation coefficients conformed with the theoretical correlations expected assuming polygenic inheritance ; 2 ) the husband-wife correlations indicate a high degree of assortative mating for skin color , but despite this effect the parent-offspring and sibling correlation coefficients are lower that the values expected under the influence of autosomal genes ; 3 ) estimates of heritability and components of phenotypic expression indicate that about 55 % of the total variability in skin reflectance could be attributed to the influence of additive genetic factors ; and 4 ) there is no evidence of X-linkage in the inheritance of skin color .
	manualset3
166816	28	412671	7	NULL	NULL	0	NULL	 skin color	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study indicates that 1 ) the parent-offspring and sibling correlation coefficients conformed with the theoretical correlations expected assuming polygenic inheritance ; 2 ) the husband-wife correlations indicate a high degree of assortative mating for skin color , but despite this effect the parent-offspring and sibling correlation coefficients are lower that the values expected under the influence of autosomal genes ; 3 ) estimates of heritability and components of phenotypic expression indicate that about 55 % of the total variability in skin reflectance could be attributed to the influence of additive genetic factors ; and 4 ) there is no evidence of X-linkage in the inheritance of skin color .
	manualset3
166817	1	412672	7	NULL	NULL	0	NULL	Accurate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Accurate in vivo monitoring of glucose concentration would be a valuable asset , particularly for management of diabetes and preterm infants during critical care .
	manualset3
166818	2	412672	7	NULL	NULL	0	NULL	in vivo monitoring	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Accurate in vivo monitoring of glucose concentration would be a valuable asset , particularly for management of diabetes and preterm infants during critical care .
	manualset3
166819	3	412672	7	NULL	NULL	0	NULL	glucose concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Accurate in vivo monitoring of glucose concentration would be a valuable asset , particularly for management of diabetes and preterm infants during critical care .
	manualset3
166820	4	412672	7	NULL	NULL	0	NULL	valuable asset	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Accurate in vivo monitoring of glucose concentration would be a valuable asset , particularly for management of diabetes and preterm infants during critical care .
	manualset3
166821	5	412672	7	NULL	NULL	0	NULL	management 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Accurate in vivo monitoring of glucose concentration would be a valuable asset , particularly for management of diabetes and preterm infants during critical care .
	manualset3
166822	6	412672	7	NULL	NULL	0	NULL	diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Accurate in vivo monitoring of glucose concentration would be a valuable asset , particularly for management of diabetes and preterm infants during critical care .
	manualset3
166823	7	412672	7	NULL	NULL	0	NULL	preterm infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Accurate in vivo monitoring of glucose concentration would be a valuable asset , particularly for management of diabetes and preterm infants during critical care .
	manualset3
166824	8	412672	7	NULL	NULL	0	NULL	critical care 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Accurate in vivo monitoring of glucose concentration would be a valuable asset , particularly for management of diabetes and preterm infants during critical care .
	manualset3
166825	1	412673	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study is based on simulated data to allow a comparison of the results of the different algorithms with true ( noise - and error-free ) marker locations .
	manualset3
166826	2	412673	7	NULL	NULL	0	NULL	simulated data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The study is based on simulated data to allow a comparison of the results of the different algorithms with true ( noise - and error-free ) marker locations .
	manualset3
166827	3	412673	7	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The study is based on simulated data to allow a comparison of the results of the different algorithms with true ( noise - and error-free ) marker locations .
	manualset3
166828	4	412673	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study is based on simulated data to allow a comparison of the results of the different algorithms with true ( noise - and error-free ) marker locations .
	manualset3
166829	5	412673	7	NULL	NULL	0	NULL	algorithms	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The study is based on simulated data to allow a comparison of the results of the different algorithms with true ( noise - and error-free ) marker locations .
	manualset3
166830	6	412673	7	NULL	NULL	0	NULL	true marker locations	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study is based on simulated data to allow a comparison of the results of the different algorithms with true ( noise - and error-free ) marker locations .
	manualset3
166832	1	412674	7	NULL	NULL	0	NULL	study material	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The study material consisted of 3 , 586 mandibles from 2 , 548 red deer and 1 , 038 fallow deer shot during sport hunting , herd management culls , and programs for population control between 1988 and 1997 ( period 1 ) and 2002 and 2009 ( period 2 ) in eastern Sierra Morena , southern Spain .
	manualset3
166833	2	412674	7	NULL	NULL	0	NULL	3 , 586	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The study material consisted of 3 , 586 mandibles from 2 , 548 red deer and 1 , 038 fallow deer shot during sport hunting , herd management culls , and programs for population control between 1988 and 1997 ( period 1 ) and 2002 and 2009 ( period 2 ) in eastern Sierra Morena , southern Spain .
	manualset3
166834	3	412674	7	NULL	NULL	0	NULL	mandibles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The study material consisted of 3 , 586 mandibles from 2 , 548 red deer and 1 , 038 fallow deer shot during sport hunting , herd management culls , and programs for population control between 1988 and 1997 ( period 1 ) and 2002 and 2009 ( period 2 ) in eastern Sierra Morena , southern Spain .
	manualset3
166835	4	412674	7	NULL	NULL	0	NULL	2 , 548	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The study material consisted of 3 , 586 mandibles from 2 , 548 red deer and 1 , 038 fallow deer shot during sport hunting , herd management culls , and programs for population control between 1988 and 1997 ( period 1 ) and 2002 and 2009 ( period 2 ) in eastern Sierra Morena , southern Spain .
	manualset3
166836	5	412674	7	NULL	NULL	0	NULL	red deer	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The study material consisted of 3 , 586 mandibles from 2 , 548 red deer and 1 , 038 fallow deer shot during sport hunting , herd management culls , and programs for population control between 1988 and 1997 ( period 1 ) and 2002 and 2009 ( period 2 ) in eastern Sierra Morena , southern Spain .
	manualset3
166837	6	412674	7	NULL	NULL	0	NULL	1 , 038	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The study material consisted of 3 , 586 mandibles from 2 , 548 red deer and 1 , 038 fallow deer shot during sport hunting , herd management culls , and programs for population control between 1988 and 1997 ( period 1 ) and 2002 and 2009 ( period 2 ) in eastern Sierra Morena , southern Spain .
	manualset3
166838	7	412674	7	NULL	NULL	0	NULL	fallow deer	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The study material consisted of 3 , 586 mandibles from 2 , 548 red deer and 1 , 038 fallow deer shot during sport hunting , herd management culls , and programs for population control between 1988 and 1997 ( period 1 ) and 2002 and 2009 ( period 2 ) in eastern Sierra Morena , southern Spain .
	manualset3
166839	8	412674	7	NULL	NULL	0	NULL	sport hunting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The study material consisted of 3 , 586 mandibles from 2 , 548 red deer and 1 , 038 fallow deer shot during sport hunting , herd management culls , and programs for population control between 1988 and 1997 ( period 1 ) and 2002 and 2009 ( period 2 ) in eastern Sierra Morena , southern Spain .
	manualset3
166840	9	412674	7	NULL	NULL	0	NULL	herd management culls	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The study material consisted of 3 , 586 mandibles from 2 , 548 red deer and 1 , 038 fallow deer shot during sport hunting , herd management culls , and programs for population control between 1988 and 1997 ( period 1 ) and 2002 and 2009 ( period 2 ) in eastern Sierra Morena , southern Spain .
	manualset3
166841	10	412674	7	NULL	NULL	0	NULL	programs	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The study material consisted of 3 , 586 mandibles from 2 , 548 red deer and 1 , 038 fallow deer shot during sport hunting , herd management culls , and programs for population control between 1988 and 1997 ( period 1 ) and 2002 and 2009 ( period 2 ) in eastern Sierra Morena , southern Spain .
	manualset3
166842	11	412674	7	NULL	NULL	0	NULL	population control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The study material consisted of 3 , 586 mandibles from 2 , 548 red deer and 1 , 038 fallow deer shot during sport hunting , herd management culls , and programs for population control between 1988 and 1997 ( period 1 ) and 2002 and 2009 ( period 2 ) in eastern Sierra Morena , southern Spain .
	manualset3
166843	12	412674	7	NULL	NULL	0	NULL	1988 and 1997	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The study material consisted of 3 , 586 mandibles from 2 , 548 red deer and 1 , 038 fallow deer shot during sport hunting , herd management culls , and programs for population control between 1988 and 1997 ( period 1 ) and 2002 and 2009 ( period 2 ) in eastern Sierra Morena , southern Spain .
	manualset3
166844	13	412674	7	NULL	NULL	0	NULL	 period 1	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The study material consisted of 3 , 586 mandibles from 2 , 548 red deer and 1 , 038 fallow deer shot during sport hunting , herd management culls , and programs for population control between 1988 and 1997 ( period 1 ) and 2002 and 2009 ( period 2 ) in eastern Sierra Morena , southern Spain .
	manualset3
166845	14	412674	7	NULL	NULL	0	NULL	 2002 and 2009	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The study material consisted of 3 , 586 mandibles from 2 , 548 red deer and 1 , 038 fallow deer shot during sport hunting , herd management culls , and programs for population control between 1988 and 1997 ( period 1 ) and 2002 and 2009 ( period 2 ) in eastern Sierra Morena , southern Spain .
	manualset3
166846	15	412674	7	NULL	NULL	0	NULL	period 2	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The study material consisted of 3 , 586 mandibles from 2 , 548 red deer and 1 , 038 fallow deer shot during sport hunting , herd management culls , and programs for population control between 1988 and 1997 ( period 1 ) and 2002 and 2009 ( period 2 ) in eastern Sierra Morena , southern Spain .
	manualset3
166847	16	412674	7	NULL	NULL	0	NULL	eastern Sierra Morena	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The study material consisted of 3 , 586 mandibles from 2 , 548 red deer and 1 , 038 fallow deer shot during sport hunting , herd management culls , and programs for population control between 1988 and 1997 ( period 1 ) and 2002 and 2009 ( period 2 ) in eastern Sierra Morena , southern Spain .
	manualset3
166848	17	412674	7	NULL	NULL	0	NULL	southern Spain	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The study material consisted of 3 , 586 mandibles from 2 , 548 red deer and 1 , 038 fallow deer shot during sport hunting , herd management culls , and programs for population control between 1988 and 1997 ( period 1 ) and 2002 and 2009 ( period 2 ) in eastern Sierra Morena , southern Spain .
	manualset3
166849	1	412675	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of neonatal alterations of behavior , BAER conduction time , and cry characteristics in infants with hyperbilirubinemia lends support to the hypothesis that low levels of bilirubin result in neonatal neurobehavioral changes that can be easily measured and recorded by these techniques .
	manualset3
166850	2	412675	7	NULL	NULL	NULL	NULL	neonatal alterations of behavior	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study of neonatal alterations of behavior , BAER conduction time , and cry characteristics in infants with hyperbilirubinemia lends support to the hypothesis that low levels of bilirubin result in neonatal neurobehavioral changes that can be easily measured and recorded by these techniques .
	manualset3
166852	4	412675	7	NULL	NULL	0	NULL	BAER conduction time	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of neonatal alterations of behavior , BAER conduction time , and cry characteristics in infants with hyperbilirubinemia lends support to the hypothesis that low levels of bilirubin result in neonatal neurobehavioral changes that can be easily measured and recorded by these techniques .
	manualset3
166853	5	412675	7	NULL	NULL	0	NULL	cry characteristics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of neonatal alterations of behavior , BAER conduction time , and cry characteristics in infants with hyperbilirubinemia lends support to the hypothesis that low levels of bilirubin result in neonatal neurobehavioral changes that can be easily measured and recorded by these techniques .
	manualset3
166854	6	412675	7	NULL	NULL	0	NULL	infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of neonatal alterations of behavior , BAER conduction time , and cry characteristics in infants with hyperbilirubinemia lends support to the hypothesis that low levels of bilirubin result in neonatal neurobehavioral changes that can be easily measured and recorded by these techniques .
	manualset3
166855	7	412675	7	NULL	NULL	0	NULL	hyperbilirubinemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of neonatal alterations of behavior , BAER conduction time , and cry characteristics in infants with hyperbilirubinemia lends support to the hypothesis that low levels of bilirubin result in neonatal neurobehavioral changes that can be easily measured and recorded by these techniques .
	manualset3
166856	8	412675	7	NULL	NULL	0	NULL	support 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of neonatal alterations of behavior , BAER conduction time , and cry characteristics in infants with hyperbilirubinemia lends support to the hypothesis that low levels of bilirubin result in neonatal neurobehavioral changes that can be easily measured and recorded by these techniques .
	manualset3
166857	9	412675	7	NULL	NULL	0	NULL	hypothesis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of neonatal alterations of behavior , BAER conduction time , and cry characteristics in infants with hyperbilirubinemia lends support to the hypothesis that low levels of bilirubin result in neonatal neurobehavioral changes that can be easily measured and recorded by these techniques .
	manualset3
166858	10	412675	7	NULL	NULL	0	NULL	low levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of neonatal alterations of behavior , BAER conduction time , and cry characteristics in infants with hyperbilirubinemia lends support to the hypothesis that low levels of bilirubin result in neonatal neurobehavioral changes that can be easily measured and recorded by these techniques .
	manualset3
166859	11	412675	7	NULL	NULL	0	NULL	 bilirubin 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of neonatal alterations of behavior , BAER conduction time , and cry characteristics in infants with hyperbilirubinemia lends support to the hypothesis that low levels of bilirubin result in neonatal neurobehavioral changes that can be easily measured and recorded by these techniques .
	manualset3
166860	12	412675	7	NULL	NULL	0	NULL	neonatal neurobehavioral changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of neonatal alterations of behavior , BAER conduction time , and cry characteristics in infants with hyperbilirubinemia lends support to the hypothesis that low levels of bilirubin result in neonatal neurobehavioral changes that can be easily measured and recorded by these techniques .
	manualset3
166861	13	412675	7	NULL	NULL	0	NULL	techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of neonatal alterations of behavior , BAER conduction time , and cry characteristics in infants with hyperbilirubinemia lends support to the hypothesis that low levels of bilirubin result in neonatal neurobehavioral changes that can be easily measured and recorded by these techniques .
	manualset3
166862	1	412676	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of the kidneys using I-131-hippuran ) .
	manualset3
166863	2	412676	7	NULL	NULL	0	NULL	kidneys	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of the kidneys using I-131-hippuran ) .
	manualset3
166864	3	412676	7	NULL	NULL	0	NULL	I-131-hippuran	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of the kidneys using I-131-hippuran ) .
	manualset3
166865	1	412677	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of these animals shows that the formation of myelin is considerably less sensitive to molecular alterations than the maintenance of myelin .
	manualset3
166866	2	412677	7	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of these animals shows that the formation of myelin is considerably less sensitive to molecular alterations than the maintenance of myelin .
	manualset3
166867	3	412677	7	NULL	NULL	0	NULL	formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of these animals shows that the formation of myelin is considerably less sensitive to molecular alterations than the maintenance of myelin .
	manualset3
166868	4	412677	7	NULL	NULL	0	NULL	myelin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of these animals shows that the formation of myelin is considerably less sensitive to molecular alterations than the maintenance of myelin .
	manualset3
166869	5	412677	7	NULL	NULL	0	NULL	molecular alterations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of these animals shows that the formation of myelin is considerably less sensitive to molecular alterations than the maintenance of myelin .
	manualset3
166870	6	412677	7	NULL	NULL	0	NULL	 maintenance	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of these animals shows that the formation of myelin is considerably less sensitive to molecular alterations than the maintenance of myelin .
	manualset3
166871	7	412677	7	NULL	NULL	0	NULL	myelin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of these animals shows that the formation of myelin is considerably less sensitive to molecular alterations than the maintenance of myelin .
	manualset3
166872	1	412678	7	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of these unusual systems promises to provide insight into many basic evolutionary questions , including the maintenance of sex , the expression of sexual conflict and kin conflict and the evolution of cheating in asexual lineages .
	manualset3
166873	2	412678	7	NULL	NULL	NULL	NULL	unusual systems	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study of these unusual systems promises to provide insight into many basic evolutionary questions , including the maintenance of sex , the expression of sexual conflict and kin conflict and the evolution of cheating in asexual lineages .
	manualset3
166874	3	412678	7	NULL	NULL	NULL	NULL	basic evolutionary questions	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study of these unusual systems promises to provide insight into many basic evolutionary questions , including the maintenance of sex , the expression of sexual conflict and kin conflict and the evolution of cheating in asexual lineages .
	manualset3
166875	4	412678	7	NULL	NULL	0	NULL	maintenance of sex	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of these unusual systems promises to provide insight into many basic evolutionary questions , including the maintenance of sex , the expression of sexual conflict and kin conflict and the evolution of cheating in asexual lineages .
	manualset3
166876	5	412678	7	NULL	NULL	0	NULL	expression of sexual conflict	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of these unusual systems promises to provide insight into many basic evolutionary questions , including the maintenance of sex , the expression of sexual conflict and kin conflict and the evolution of cheating in asexual lineages .
	manualset3
166877	6	412678	7	NULL	NULL	0	NULL	kin conflict 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of these unusual systems promises to provide insight into many basic evolutionary questions , including the maintenance of sex , the expression of sexual conflict and kin conflict and the evolution of cheating in asexual lineages .
	manualset3
166878	7	412678	7	NULL	NULL	0	NULL	evolution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of these unusual systems promises to provide insight into many basic evolutionary questions , including the maintenance of sex , the expression of sexual conflict and kin conflict and the evolution of cheating in asexual lineages .
	manualset3
166879	8	412678	7	NULL	NULL	0	NULL	cheating	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of these unusual systems promises to provide insight into many basic evolutionary questions , including the maintenance of sex , the expression of sexual conflict and kin conflict and the evolution of cheating in asexual lineages .
	manualset3
166880	9	412678	7	NULL	NULL	0	NULL	asexual lineages 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of these unusual systems promises to provide insight into many basic evolutionary questions , including the maintenance of sex , the expression of sexual conflict and kin conflict and the evolution of cheating in asexual lineages .
	manualset3
169199	10	412678	7	NULL	NULL	0	NULL	insight	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of these unusual systems promises to provide insight into many basic evolutionary questions , including the maintenance of sex , the expression of sexual conflict and kin conflict and the evolution of cheating in asexual lineages .
	manualset3
166881	1	412679	7	NULL	NULL	0	NULL	study population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The study population was categorized into groups according to cigarette smoking experience and subgroups according to age and number of pack-years of exposure .
	manualset3
166882	2	412679	7	NULL	NULL	0	NULL	 groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The study population was categorized into groups according to cigarette smoking experience and subgroups according to age and number of pack-years of exposure .
	manualset3
166883	3	412679	7	NULL	NULL	0	NULL	cigarette smoking experience	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study population was categorized into groups according to cigarette smoking experience and subgroups according to age and number of pack-years of exposure .
	manualset3
166884	4	412679	7	NULL	NULL	0	NULL	subgroups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The study population was categorized into groups according to cigarette smoking experience and subgroups according to age and number of pack-years of exposure .
	manualset3
166885	5	412679	7	NULL	NULL	0	NULL	age	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The study population was categorized into groups according to cigarette smoking experience and subgroups according to age and number of pack-years of exposure .
	manualset3
166886	6	412679	7	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study population was categorized into groups according to cigarette smoking experience and subgroups according to age and number of pack-years of exposure .
	manualset3
166887	7	412679	7	NULL	NULL	0	NULL	pack-years of exposure	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The study population was categorized into groups according to cigarette smoking experience and subgroups according to age and number of pack-years of exposure .
	manualset3
166888	1	412680	7	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study provides useful information on the prevalence and management protocols of childhood cancer in this part of eastern India .
	manualset3
166889	2	412680	7	NULL	NULL	0	NULL	information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The study provides useful information on the prevalence and management protocols of childhood cancer in this part of eastern India .
	manualset3
166890	3	412680	7	NULL	NULL	0	NULL	prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study provides useful information on the prevalence and management protocols of childhood cancer in this part of eastern India .
	manualset3
166891	4	412680	7	NULL	NULL	0	NULL	management protocols	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study provides useful information on the prevalence and management protocols of childhood cancer in this part of eastern India .
	manualset3
166892	5	412680	7	NULL	NULL	0	NULL	childhood cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The study provides useful information on the prevalence and management protocols of childhood cancer in this part of eastern India .
	manualset3
166893	6	412680	7	NULL	NULL	0	NULL	part of eastern India	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The study provides useful information on the prevalence and management protocols of childhood cancer in this part of eastern India .
	manualset3
166894	1	412681	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study revealed important insights into the possible role of the intervening spacer region in cellular protein binding and influencing internal initiation of translation of CVB3 RNA .
	manualset3
166895	2	412681	7	NULL	NULL	NULL	NULL	insights	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study revealed important insights into the possible role of the intervening spacer region in cellular protein binding and influencing internal initiation of translation of CVB3 RNA .
	manualset3
166896	3	412681	7	NULL	NULL	NULL	NULL	role	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study revealed important insights into the possible role of the intervening spacer region in cellular protein binding and influencing internal initiation of translation of CVB3 RNA .
	manualset3
166897	4	412681	7	NULL	NULL	0	NULL	 intervening spacer region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The study revealed important insights into the possible role of the intervening spacer region in cellular protein binding and influencing internal initiation of translation of CVB3 RNA .
	manualset3
166898	5	412681	7	NULL	NULL	0	NULL	cellular protein binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The study revealed important insights into the possible role of the intervening spacer region in cellular protein binding and influencing internal initiation of translation of CVB3 RNA .
	manualset3
166899	6	412681	7	NULL	NULL	0	NULL	internal initiation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The study revealed important insights into the possible role of the intervening spacer region in cellular protein binding and influencing internal initiation of translation of CVB3 RNA .
	manualset3
166900	7	412681	7	NULL	NULL	0	NULL	translation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The study revealed important insights into the possible role of the intervening spacer region in cellular protein binding and influencing internal initiation of translation of CVB3 RNA .
	manualset3
166901	8	412681	7	NULL	NULL	0	NULL	 CVB3 RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The study revealed important insights into the possible role of the intervening spacer region in cellular protein binding and influencing internal initiation of translation of CVB3 RNA .
	manualset3
166902	1	412682	7	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study showed that the resistance to nystatin has been rising in these organisms with years .
	manualset3
166903	2	412682	7	NULL	NULL	0	NULL	resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The study showed that the resistance to nystatin has been rising in these organisms with years .
	manualset3
166904	3	412682	7	NULL	NULL	0	NULL	nystatin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The study showed that the resistance to nystatin has been rising in these organisms with years .
	manualset3
166905	4	412682	7	NULL	NULL	0	NULL	organisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The study showed that the resistance to nystatin has been rising in these organisms with years .
	manualset3
166906	5	412682	7	NULL	NULL	0	NULL	years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The study showed that the resistance to nystatin has been rising in these organisms with years .
	manualset3
166907	1	412683	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study suggests albumin can cause segregation of protein bound-lipid domains in surfactant at NMR timescales ( 10 ( -5 ) s ) .
	manualset3
166908	2	412683	7	NULL	NULL	0	NULL	albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The study suggests albumin can cause segregation of protein bound-lipid domains in surfactant at NMR timescales ( 10 ( -5 ) s ) .
	manualset3
166909	3	412683	7	NULL	NULL	NULL	NULL	segregation 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study suggests albumin can cause segregation of protein bound-lipid domains in surfactant at NMR timescales ( 10 ( -5 ) s ) .
	manualset3
166910	4	412683	7	NULL	NULL	0	NULL	protein bound-lipid domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The study suggests albumin can cause segregation of protein bound-lipid domains in surfactant at NMR timescales ( 10 ( -5 ) s ) .
	manualset3
166911	5	412683	7	NULL	NULL	NULL	NULL	surfactant	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The study suggests albumin can cause segregation of protein bound-lipid domains in surfactant at NMR timescales ( 10 ( -5 ) s ) .
	manualset3
166912	6	412683	7	NULL	NULL	0	NULL	NMR timescales	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study suggests albumin can cause segregation of protein bound-lipid domains in surfactant at NMR timescales ( 10 ( -5 ) s ) .
	manualset3
166913	7	412683	7	NULL	NULL	0	NULL	10 ( -5 ) s	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The study suggests albumin can cause segregation of protein bound-lipid domains in surfactant at NMR timescales ( 10 ( -5 ) s ) .
	manualset3
166914	1	412684	7	NULL	NULL	0	NULL	Accurate method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Accurate method to study static volume-pressure relationships in small fetal and neonatal animals .
	manualset3
166915	2	412684	7	NULL	NULL	0	NULL	static volume-pressure relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Accurate method to study static volume-pressure relationships in small fetal and neonatal animals .
	manualset3
166916	3	412684	7	NULL	NULL	0	NULL	small fetal animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Accurate method to study static volume-pressure relationships in small fetal and neonatal animals .
	manualset3
166917	4	412684	7	NULL	NULL	0	NULL	neonatal animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Accurate method to study static volume-pressure relationships in small fetal and neonatal animals .
	manualset3
166918	1	412685	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study suggests that a drug which affects both eating behavior and mouse killing is more effective in determining behavioral outcomes than a drug which affects only mouse killing .
	manualset3
166919	2	412685	7	NULL	NULL	0	NULL	 drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The study suggests that a drug which affects both eating behavior and mouse killing is more effective in determining behavioral outcomes than a drug which affects only mouse killing .
	manualset3
166920	3	412685	7	NULL	NULL	0	NULL	eating behavior	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study suggests that a drug which affects both eating behavior and mouse killing is more effective in determining behavioral outcomes than a drug which affects only mouse killing .
	manualset3
166921	4	412685	7	NULL	NULL	0	NULL	mouse killing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The study suggests that a drug which affects both eating behavior and mouse killing is more effective in determining behavioral outcomes than a drug which affects only mouse killing .
	manualset3
166922	5	412685	7	NULL	NULL	0	NULL	behavioral outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study suggests that a drug which affects both eating behavior and mouse killing is more effective in determining behavioral outcomes than a drug which affects only mouse killing .
	manualset3
166923	6	412685	7	NULL	NULL	0	NULL	 drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The study suggests that a drug which affects both eating behavior and mouse killing is more effective in determining behavioral outcomes than a drug which affects only mouse killing .
	manualset3
166924	7	412685	7	NULL	NULL	0	NULL	mouse killing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The study suggests that a drug which affects both eating behavior and mouse killing is more effective in determining behavioral outcomes than a drug which affects only mouse killing .
	manualset3
166925	1	412686	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was aimed to investigate the expression of VEGF mRNA and VEGF protein in HL-60 cells treated with diallyl disulfide ( DADS ) , and to explore the antileukemic mechanism of DADS in respect of VEGF production .
	manualset3
166926	2	412686	7	NULL	NULL	0	NULL	 expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was aimed to investigate the expression of VEGF mRNA and VEGF protein in HL-60 cells treated with diallyl disulfide ( DADS ) , and to explore the antileukemic mechanism of DADS in respect of VEGF production .
	manualset3
166927	3	412686	7	NULL	NULL	0	NULL	VEGF mRNA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was aimed to investigate the expression of VEGF mRNA and VEGF protein in HL-60 cells treated with diallyl disulfide ( DADS ) , and to explore the antileukemic mechanism of DADS in respect of VEGF production .
	manualset3
166928	4	412686	7	NULL	NULL	0	NULL	VEGF protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was aimed to investigate the expression of VEGF mRNA and VEGF protein in HL-60 cells treated with diallyl disulfide ( DADS ) , and to explore the antileukemic mechanism of DADS in respect of VEGF production .
	manualset3
166929	5	412686	7	NULL	NULL	0	NULL	HL-60 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was aimed to investigate the expression of VEGF mRNA and VEGF protein in HL-60 cells treated with diallyl disulfide ( DADS ) , and to explore the antileukemic mechanism of DADS in respect of VEGF production .
	manualset3
166930	6	412686	7	NULL	NULL	0	NULL	diallyl disulfide ( DADS )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was aimed to investigate the expression of VEGF mRNA and VEGF protein in HL-60 cells treated with diallyl disulfide ( DADS ) , and to explore the antileukemic mechanism of DADS in respect of VEGF production .
	manualset3
166931	7	412686	7	NULL	NULL	0	NULL	antileukemic mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was aimed to investigate the expression of VEGF mRNA and VEGF protein in HL-60 cells treated with diallyl disulfide ( DADS ) , and to explore the antileukemic mechanism of DADS in respect of VEGF production .
	manualset3
166932	8	412686	7	NULL	NULL	0	NULL	DADS	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was aimed to investigate the expression of VEGF mRNA and VEGF protein in HL-60 cells treated with diallyl disulfide ( DADS ) , and to explore the antileukemic mechanism of DADS in respect of VEGF production .
	manualset3
166933	9	412686	7	NULL	NULL	0	NULL	VEGF production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was aimed to investigate the expression of VEGF mRNA and VEGF protein in HL-60 cells treated with diallyl disulfide ( DADS ) , and to explore the antileukemic mechanism of DADS in respect of VEGF production .
	manualset3
166934	1	412687	7	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was conducted on 14 patients with moderate CP ( group 1 ) and 14 patients with severe CP ( group 2 ) .
	manualset3
166935	2	412687	7	NULL	NULL	0	NULL	14 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was conducted on 14 patients with moderate CP ( group 1 ) and 14 patients with severe CP ( group 2 ) .
	manualset3
166936	3	412687	7	NULL	NULL	0	NULL	moderate CP ( group 1 )	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was conducted on 14 patients with moderate CP ( group 1 ) and 14 patients with severe CP ( group 2 ) .
	manualset3
166937	4	412687	7	NULL	NULL	0	NULL	14 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was conducted on 14 patients with moderate CP ( group 1 ) and 14 patients with severe CP ( group 2 ) .
	manualset3
166938	5	412687	7	NULL	NULL	0	NULL	severe CP ( group 2 )	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was conducted on 14 patients with moderate CP ( group 1 ) and 14 patients with severe CP ( group 2 ) .
	manualset3
166939	1	412688	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was performed on 10 adults ( age range , 15-40 yr ) whose lungs were mechanically ventilated ( air/O2 ) and who were sedated ( phenoperidine , 1 mg/h ) , and was conducted using a radial artery cannula ; a 7.5-Fr , thermodilution , flow-directed , pulmonary artery catheter ; an intraventricular catheter ; and a catheter in the jugular venous bulb .
	manualset3
166940	2	412688	7	NULL	NULL	0	NULL	10 adults 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was performed on 10 adults ( age range , 15-40 yr ) whose lungs were mechanically ventilated ( air/O2 ) and who were sedated ( phenoperidine , 1 mg/h ) , and was conducted using a radial artery cannula ; a 7.5-Fr , thermodilution , flow-directed , pulmonary artery catheter ; an intraventricular catheter ; and a catheter in the jugular venous bulb .
	manualset3
166941	3	412688	7	NULL	NULL	0	NULL	age range	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was performed on 10 adults ( age range , 15-40 yr ) whose lungs were mechanically ventilated ( air/O2 ) and who were sedated ( phenoperidine , 1 mg/h ) , and was conducted using a radial artery cannula ; a 7.5-Fr , thermodilution , flow-directed , pulmonary artery catheter ; an intraventricular catheter ; and a catheter in the jugular venous bulb .
	manualset3
166942	4	412688	7	NULL	NULL	0	NULL	15-40 yr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was performed on 10 adults ( age range , 15-40 yr ) whose lungs were mechanically ventilated ( air/O2 ) and who were sedated ( phenoperidine , 1 mg/h ) , and was conducted using a radial artery cannula ; a 7.5-Fr , thermodilution , flow-directed , pulmonary artery catheter ; an intraventricular catheter ; and a catheter in the jugular venous bulb .
	manualset3
166943	5	412688	7	NULL	NULL	0	NULL	 lungs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was performed on 10 adults ( age range , 15-40 yr ) whose lungs were mechanically ventilated ( air/O2 ) and who were sedated ( phenoperidine , 1 mg/h ) , and was conducted using a radial artery cannula ; a 7.5-Fr , thermodilution , flow-directed , pulmonary artery catheter ; an intraventricular catheter ; and a catheter in the jugular venous bulb .
	manualset3
166944	6	412688	7	NULL	NULL	0	NULL	mechanically ventilated ( air/O2 ) 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was performed on 10 adults ( age range , 15-40 yr ) whose lungs were mechanically ventilated ( air/O2 ) and who were sedated ( phenoperidine , 1 mg/h ) , and was conducted using a radial artery cannula ; a 7.5-Fr , thermodilution , flow-directed , pulmonary artery catheter ; an intraventricular catheter ; and a catheter in the jugular venous bulb .
	manualset3
166945	7	412688	7	NULL	NULL	0	NULL	sedated	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was performed on 10 adults ( age range , 15-40 yr ) whose lungs were mechanically ventilated ( air/O2 ) and who were sedated ( phenoperidine , 1 mg/h ) , and was conducted using a radial artery cannula ; a 7.5-Fr , thermodilution , flow-directed , pulmonary artery catheter ; an intraventricular catheter ; and a catheter in the jugular venous bulb .
	manualset3
166946	8	412688	7	NULL	NULL	0	NULL	phenoperidine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was performed on 10 adults ( age range , 15-40 yr ) whose lungs were mechanically ventilated ( air/O2 ) and who were sedated ( phenoperidine , 1 mg/h ) , and was conducted using a radial artery cannula ; a 7.5-Fr , thermodilution , flow-directed , pulmonary artery catheter ; an intraventricular catheter ; and a catheter in the jugular venous bulb .
	manualset3
166947	9	412688	7	NULL	NULL	0	NULL	1 mg/h	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was performed on 10 adults ( age range , 15-40 yr ) whose lungs were mechanically ventilated ( air/O2 ) and who were sedated ( phenoperidine , 1 mg/h ) , and was conducted using a radial artery cannula ; a 7.5-Fr , thermodilution , flow-directed , pulmonary artery catheter ; an intraventricular catheter ; and a catheter in the jugular venous bulb .
	manualset3
166948	10	412688	7	NULL	NULL	0	NULL	radial artery cannula	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was performed on 10 adults ( age range , 15-40 yr ) whose lungs were mechanically ventilated ( air/O2 ) and who were sedated ( phenoperidine , 1 mg/h ) , and was conducted using a radial artery cannula ; a 7.5-Fr , thermodilution , flow-directed , pulmonary artery catheter ; an intraventricular catheter ; and a catheter in the jugular venous bulb .
	manualset3
166949	11	412688	7	NULL	NULL	0	NULL	7.5-Fr	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was performed on 10 adults ( age range , 15-40 yr ) whose lungs were mechanically ventilated ( air/O2 ) and who were sedated ( phenoperidine , 1 mg/h ) , and was conducted using a radial artery cannula ; a 7.5-Fr , thermodilution , flow-directed , pulmonary artery catheter ; an intraventricular catheter ; and a catheter in the jugular venous bulb .
	manualset3
166950	12	412688	7	NULL	NULL	0	NULL	 thermodilution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was performed on 10 adults ( age range , 15-40 yr ) whose lungs were mechanically ventilated ( air/O2 ) and who were sedated ( phenoperidine , 1 mg/h ) , and was conducted using a radial artery cannula ; a 7.5-Fr , thermodilution , flow-directed , pulmonary artery catheter ; an intraventricular catheter ; and a catheter in the jugular venous bulb .
	manualset3
166951	13	412688	7	NULL	NULL	0	NULL	flow-directed , pulmonary artery catheter	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was performed on 10 adults ( age range , 15-40 yr ) whose lungs were mechanically ventilated ( air/O2 ) and who were sedated ( phenoperidine , 1 mg/h ) , and was conducted using a radial artery cannula ; a 7.5-Fr , thermodilution , flow-directed , pulmonary artery catheter ; an intraventricular catheter ; and a catheter in the jugular venous bulb .
	manualset3
166952	14	412688	7	NULL	NULL	0	NULL	intraventricular catheter	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was performed on 10 adults ( age range , 15-40 yr ) whose lungs were mechanically ventilated ( air/O2 ) and who were sedated ( phenoperidine , 1 mg/h ) , and was conducted using a radial artery cannula ; a 7.5-Fr , thermodilution , flow-directed , pulmonary artery catheter ; an intraventricular catheter ; and a catheter in the jugular venous bulb .
	manualset3
166953	15	412688	7	NULL	NULL	0	NULL	catheter	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was performed on 10 adults ( age range , 15-40 yr ) whose lungs were mechanically ventilated ( air/O2 ) and who were sedated ( phenoperidine , 1 mg/h ) , and was conducted using a radial artery cannula ; a 7.5-Fr , thermodilution , flow-directed , pulmonary artery catheter ; an intraventricular catheter ; and a catheter in the jugular venous bulb .
	manualset3
166954	16	412688	7	NULL	NULL	0	NULL	jugular venous bulb	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was performed on 10 adults ( age range , 15-40 yr ) whose lungs were mechanically ventilated ( air/O2 ) and who were sedated ( phenoperidine , 1 mg/h ) , and was conducted using a radial artery cannula ; a 7.5-Fr , thermodilution , flow-directed , pulmonary artery catheter ; an intraventricular catheter ; and a catheter in the jugular venous bulb .
	manualset3
166955	1	412689	7	NULL	NULL	0	NULL	 subcutaneous injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The subcutaneous injection of arachidonic acid ( 200-400 mg/kg per day ) into pregnant diabetic rats during the period of organ differentiation ( days 6-12 ) did not alter the maternal glucose concentration , the maternal weight gain , or the weight of the embryos .
	manualset3
166956	2	412689	7	NULL	NULL	0	NULL	arachidonic acid	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The subcutaneous injection of arachidonic acid ( 200-400 mg/kg per day ) into pregnant diabetic rats during the period of organ differentiation ( days 6-12 ) did not alter the maternal glucose concentration , the maternal weight gain , or the weight of the embryos .
	manualset3
166957	3	412689	7	NULL	NULL	0	NULL	200-400 mg/kg per day	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The subcutaneous injection of arachidonic acid ( 200-400 mg/kg per day ) into pregnant diabetic rats during the period of organ differentiation ( days 6-12 ) did not alter the maternal glucose concentration , the maternal weight gain , or the weight of the embryos .
	manualset3
166958	4	412689	7	NULL	NULL	0	NULL	pregnant diabetic rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The subcutaneous injection of arachidonic acid ( 200-400 mg/kg per day ) into pregnant diabetic rats during the period of organ differentiation ( days 6-12 ) did not alter the maternal glucose concentration , the maternal weight gain , or the weight of the embryos .
	manualset3
166959	5	412689	7	NULL	NULL	0	NULL	period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The subcutaneous injection of arachidonic acid ( 200-400 mg/kg per day ) into pregnant diabetic rats during the period of organ differentiation ( days 6-12 ) did not alter the maternal glucose concentration , the maternal weight gain , or the weight of the embryos .
	manualset3
166960	6	412689	7	NULL	NULL	0	NULL	organ differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The subcutaneous injection of arachidonic acid ( 200-400 mg/kg per day ) into pregnant diabetic rats during the period of organ differentiation ( days 6-12 ) did not alter the maternal glucose concentration , the maternal weight gain , or the weight of the embryos .
	manualset3
166961	7	412689	7	NULL	NULL	0	NULL	days 6-12	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The subcutaneous injection of arachidonic acid ( 200-400 mg/kg per day ) into pregnant diabetic rats during the period of organ differentiation ( days 6-12 ) did not alter the maternal glucose concentration , the maternal weight gain , or the weight of the embryos .
	manualset3
166962	8	412689	7	NULL	NULL	0	NULL	maternal glucose concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The subcutaneous injection of arachidonic acid ( 200-400 mg/kg per day ) into pregnant diabetic rats during the period of organ differentiation ( days 6-12 ) did not alter the maternal glucose concentration , the maternal weight gain , or the weight of the embryos .
	manualset3
166963	9	412689	7	NULL	NULL	0	NULL	maternal weight gain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The subcutaneous injection of arachidonic acid ( 200-400 mg/kg per day ) into pregnant diabetic rats during the period of organ differentiation ( days 6-12 ) did not alter the maternal glucose concentration , the maternal weight gain , or the weight of the embryos .
	manualset3
166964	10	412689	7	NULL	NULL	0	NULL	weight 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The subcutaneous injection of arachidonic acid ( 200-400 mg/kg per day ) into pregnant diabetic rats during the period of organ differentiation ( days 6-12 ) did not alter the maternal glucose concentration , the maternal weight gain , or the weight of the embryos .
	manualset3
166965	11	412689	7	NULL	NULL	0	NULL	embryos	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The subcutaneous injection of arachidonic acid ( 200-400 mg/kg per day ) into pregnant diabetic rats during the period of organ differentiation ( days 6-12 ) did not alter the maternal glucose concentration , the maternal weight gain , or the weight of the embryos .
	manualset3
166966	1	412690	7	NULL	NULL	0	NULL	subiculum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The subiculum , which generated gamma , remained at the baseline 3.0 mM .
	manualset3
166967	2	412690	7	NULL	NULL	0	NULL	gamma	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The subiculum , which generated gamma , remained at the baseline 3.0 mM .
	manualset3
166968	3	412690	7	NULL	NULL	0	NULL	baseline 3.0 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The subiculum , which generated gamma , remained at the baseline 3.0 mM .
	manualset3
166969	1	412691	7	NULL	NULL	0	NULL	subjective pain sensation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The subjective pain sensation induced by capsaicin was significantly increased in CM with respect to both MA patients and normal subjects ; the R2 area was increased in CM patients during capsaicin application , with respect to controls and MA patients , who did not exhibit any reflex alterations .
	manualset3
166970	2	412691	7	NULL	NULL	0	NULL	capsaicin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The subjective pain sensation induced by capsaicin was significantly increased in CM with respect to both MA patients and normal subjects ; the R2 area was increased in CM patients during capsaicin application , with respect to controls and MA patients , who did not exhibit any reflex alterations .
	manualset3
166971	3	412691	7	NULL	NULL	0	NULL	CM	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The subjective pain sensation induced by capsaicin was significantly increased in CM with respect to both MA patients and normal subjects ; the R2 area was increased in CM patients during capsaicin application , with respect to controls and MA patients , who did not exhibit any reflex alterations .
	manualset3
166972	4	412691	7	NULL	NULL	0	NULL	MA patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The subjective pain sensation induced by capsaicin was significantly increased in CM with respect to both MA patients and normal subjects ; the R2 area was increased in CM patients during capsaicin application , with respect to controls and MA patients , who did not exhibit any reflex alterations .
	manualset3
166973	5	412691	7	NULL	NULL	0	NULL	normal subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The subjective pain sensation induced by capsaicin was significantly increased in CM with respect to both MA patients and normal subjects ; the R2 area was increased in CM patients during capsaicin application , with respect to controls and MA patients , who did not exhibit any reflex alterations .
	manualset3
166974	6	412691	7	NULL	NULL	0	NULL	R2 area	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The subjective pain sensation induced by capsaicin was significantly increased in CM with respect to both MA patients and normal subjects ; the R2 area was increased in CM patients during capsaicin application , with respect to controls and MA patients , who did not exhibit any reflex alterations .
	manualset3
166975	7	412691	7	NULL	NULL	0	NULL	CM patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The subjective pain sensation induced by capsaicin was significantly increased in CM with respect to both MA patients and normal subjects ; the R2 area was increased in CM patients during capsaicin application , with respect to controls and MA patients , who did not exhibit any reflex alterations .
	manualset3
166976	8	412691	7	NULL	NULL	0	NULL	capsaicin application	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The subjective pain sensation induced by capsaicin was significantly increased in CM with respect to both MA patients and normal subjects ; the R2 area was increased in CM patients during capsaicin application , with respect to controls and MA patients , who did not exhibit any reflex alterations .
	manualset3
166977	9	412691	7	NULL	NULL	0	NULL	MA patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The subjective pain sensation induced by capsaicin was significantly increased in CM with respect to both MA patients and normal subjects ; the R2 area was increased in CM patients during capsaicin application , with respect to controls and MA patients , who did not exhibit any reflex alterations .
	manualset3
166978	10	412691	7	NULL	NULL	0	NULL	reflex alterations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The subjective pain sensation induced by capsaicin was significantly increased in CM with respect to both MA patients and normal subjects ; the R2 area was increased in CM patients during capsaicin application , with respect to controls and MA patients , who did not exhibit any reflex alterations .
	manualset3
166979	11	412691	7	NULL	NULL	0	NULL	controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The subjective pain sensation induced by capsaicin was significantly increased in CM with respect to both MA patients and normal subjects ; the R2 area was increased in CM patients during capsaicin application , with respect to controls and MA patients , who did not exhibit any reflex alterations .
	manualset3
166980	1	412692	7	NULL	NULL	0	NULL	subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The subjects with insulinomas had lower mean plasma glucose and higher insulin concentrations than controls , 3.6 + / - 0.3 mmol/L ( P = 0.01 ) and 150 + / - 42 pmol/L ( P = 0.01 ) , respectively .
	manualset3
166981	2	412692	7	NULL	NULL	0	NULL	 insulinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The subjects with insulinomas had lower mean plasma glucose and higher insulin concentrations than controls , 3.6 + / - 0.3 mmol/L ( P = 0.01 ) and 150 + / - 42 pmol/L ( P = 0.01 ) , respectively .
	manualset3
166982	3	412692	7	NULL	NULL	NULL	NULL	 lower mean plasma glucose	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The subjects with insulinomas had lower mean plasma glucose and higher insulin concentrations than controls , 3.6 + / - 0.3 mmol/L ( P = 0.01 ) and 150 + / - 42 pmol/L ( P = 0.01 ) , respectively .
	manualset3
166983	4	412692	7	NULL	NULL	0	NULL	higher insulin concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The subjects with insulinomas had lower mean plasma glucose and higher insulin concentrations than controls , 3.6 + / - 0.3 mmol/L ( P = 0.01 ) and 150 + / - 42 pmol/L ( P = 0.01 ) , respectively .
	manualset3
166984	5	412692	7	NULL	NULL	0	NULL	 controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The subjects with insulinomas had lower mean plasma glucose and higher insulin concentrations than controls , 3.6 + / - 0.3 mmol/L ( P = 0.01 ) and 150 + / - 42 pmol/L ( P = 0.01 ) , respectively .
	manualset3
166985	6	412692	7	NULL	NULL	0	NULL	3.6 + / - 0.3 mmol/L ( P = 0.01 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The subjects with insulinomas had lower mean plasma glucose and higher insulin concentrations than controls , 3.6 + / - 0.3 mmol/L ( P = 0.01 ) and 150 + / - 42 pmol/L ( P = 0.01 ) , respectively .
	manualset3
166986	7	412692	7	NULL	NULL	0	NULL	150 + / - 42 pmol/L ( P = 0.01 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The subjects with insulinomas had lower mean plasma glucose and higher insulin concentrations than controls , 3.6 + / - 0.3 mmol/L ( P = 0.01 ) and 150 + / - 42 pmol/L ( P = 0.01 ) , respectively .
	manualset3
166987	1	412693	7	NULL	NULL	NULL	NULL	 cell-survival curves	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The subsequent cell-survival curves were complex ; however , survival generally decreased in a time - and temperature-dependent manner during continuous heating at 33 , 37 or 42 degrees C. Constant 33 degrees C heating induced five hsp at 90 , 72 , 70 , 24 and 19 kilodaltons ( kDa ) .
	manualset3
166988	2	412693	7	NULL	NULL	0	NULL	survival 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The subsequent cell-survival curves were complex ; however , survival generally decreased in a time - and temperature-dependent manner during continuous heating at 33 , 37 or 42 degrees C. Constant 33 degrees C heating induced five hsp at 90 , 72 , 70 , 24 and 19 kilodaltons ( kDa ) .
	manualset3
166989	3	412693	7	NULL	NULL	0	NULL	 time -dependent manner	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The subsequent cell-survival curves were complex ; however , survival generally decreased in a time - and temperature-dependent manner during continuous heating at 33 , 37 or 42 degrees C. Constant 33 degrees C heating induced five hsp at 90 , 72 , 70 , 24 and 19 kilodaltons ( kDa ) .
	manualset3
166990	4	412693	7	NULL	NULL	0	NULL	temperature-dependent manner	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The subsequent cell-survival curves were complex ; however , survival generally decreased in a time - and temperature-dependent manner during continuous heating at 33 , 37 or 42 degrees C. Constant 33 degrees C heating induced five hsp at 90 , 72 , 70 , 24 and 19 kilodaltons ( kDa ) .
	manualset3
166991	5	412693	7	NULL	NULL	0	NULL	continuous heating	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The subsequent cell-survival curves were complex ; however , survival generally decreased in a time - and temperature-dependent manner during continuous heating at 33 , 37 or 42 degrees C. Constant 33 degrees C heating induced five hsp at 90 , 72 , 70 , 24 and 19 kilodaltons ( kDa ) .
	manualset3
166992	6	412693	7	NULL	NULL	0	NULL	 33 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The subsequent cell-survival curves were complex ; however , survival generally decreased in a time - and temperature-dependent manner during continuous heating at 33 , 37 or 42 degrees C. Constant 33 degrees C heating induced five hsp at 90 , 72 , 70 , 24 and 19 kilodaltons ( kDa ) .
	manualset3
166993	7	412693	7	NULL	NULL	0	NULL	 37 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The subsequent cell-survival curves were complex ; however , survival generally decreased in a time - and temperature-dependent manner during continuous heating at 33 , 37 or 42 degrees C. Constant 33 degrees C heating induced five hsp at 90 , 72 , 70 , 24 and 19 kilodaltons ( kDa ) .
	manualset3
166994	8	412693	7	NULL	NULL	0	NULL	42 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The subsequent cell-survival curves were complex ; however , survival generally decreased in a time - and temperature-dependent manner during continuous heating at 33 , 37 or 42 degrees C. Constant 33 degrees C heating induced five hsp at 90 , 72 , 70 , 24 and 19 kilodaltons ( kDa ) .
	manualset3
166995	9	412693	7	NULL	NULL	0	NULL	33 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The subsequent cell-survival curves were complex ; however , survival generally decreased in a time - and temperature-dependent manner during continuous heating at 33 , 37 or 42 degrees C. Constant 33 degrees C heating induced five hsp at 90 , 72 , 70 , 24 and 19 kilodaltons ( kDa ) .
	manualset3
166996	10	412693	7	NULL	NULL	0	NULL	heating	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The subsequent cell-survival curves were complex ; however , survival generally decreased in a time - and temperature-dependent manner during continuous heating at 33 , 37 or 42 degrees C. Constant 33 degrees C heating induced five hsp at 90 , 72 , 70 , 24 and 19 kilodaltons ( kDa ) .
	manualset3
166997	11	412693	7	NULL	NULL	0	NULL	five hsp	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The subsequent cell-survival curves were complex ; however , survival generally decreased in a time - and temperature-dependent manner during continuous heating at 33 , 37 or 42 degrees C. Constant 33 degrees C heating induced five hsp at 90 , 72 , 70 , 24 and 19 kilodaltons ( kDa ) .
	manualset3
166998	12	412693	7	NULL	NULL	0	NULL	 90 kilodaltons	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The subsequent cell-survival curves were complex ; however , survival generally decreased in a time - and temperature-dependent manner during continuous heating at 33 , 37 or 42 degrees C. Constant 33 degrees C heating induced five hsp at 90 , 72 , 70 , 24 and 19 kilodaltons ( kDa ) .
	manualset3
166999	13	412693	7	NULL	NULL	0	NULL	72 kilodaltons	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The subsequent cell-survival curves were complex ; however , survival generally decreased in a time - and temperature-dependent manner during continuous heating at 33 , 37 or 42 degrees C. Constant 33 degrees C heating induced five hsp at 90 , 72 , 70 , 24 and 19 kilodaltons ( kDa ) .
	manualset3
167000	14	412693	7	NULL	NULL	0	NULL	70 kilodaltons	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The subsequent cell-survival curves were complex ; however , survival generally decreased in a time - and temperature-dependent manner during continuous heating at 33 , 37 or 42 degrees C. Constant 33 degrees C heating induced five hsp at 90 , 72 , 70 , 24 and 19 kilodaltons ( kDa ) .
	manualset3
167001	15	412693	7	NULL	NULL	0	NULL	24 kilodaltons	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The subsequent cell-survival curves were complex ; however , survival generally decreased in a time - and temperature-dependent manner during continuous heating at 33 , 37 or 42 degrees C. Constant 33 degrees C heating induced five hsp at 90 , 72 , 70 , 24 and 19 kilodaltons ( kDa ) .
	manualset3
167002	16	412693	7	NULL	NULL	0	NULL	19 kilodaltons	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The subsequent cell-survival curves were complex ; however , survival generally decreased in a time - and temperature-dependent manner during continuous heating at 33 , 37 or 42 degrees C. Constant 33 degrees C heating induced five hsp at 90 , 72 , 70 , 24 and 19 kilodaltons ( kDa ) .
	manualset3
167003	17	412693	7	NULL	NULL	0	NULL	kDa	Unit												NULL		0	NULL	NULL	NULL	NULL	NULL	The subsequent cell-survival curves were complex ; however , survival generally decreased in a time - and temperature-dependent manner during continuous heating at 33 , 37 or 42 degrees C. Constant 33 degrees C heating induced five hsp at 90 , 72 , 70 , 24 and 19 kilodaltons ( kDa ) .
	manualset3
167004	1	412694	7	NULL	NULL	0	NULL	 incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The subsequent incidence of distant metastases was not increased by the use of Ro-07-0582 at the time of `` primary '' tumor irradiation .
	manualset3
167005	2	412694	7	NULL	NULL	0	NULL	distant metastases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The subsequent incidence of distant metastases was not increased by the use of Ro-07-0582 at the time of `` primary '' tumor irradiation .
	manualset3
167006	3	412694	7	NULL	NULL	0	NULL	Ro-07-0582	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The subsequent incidence of distant metastases was not increased by the use of Ro-07-0582 at the time of `` primary '' tumor irradiation .
	manualset3
167007	4	412694	7	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The subsequent incidence of distant metastases was not increased by the use of Ro-07-0582 at the time of `` primary '' tumor irradiation .
	manualset3
167008	5	412694	7	NULL	NULL	0	NULL	`` primary '' tumor irradiation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The subsequent incidence of distant metastases was not increased by the use of Ro-07-0582 at the time of `` primary '' tumor irradiation .
	manualset3
167009	1	412695	7	NULL	NULL	0	NULL	substrate specificities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The substrate specificities of folylpolyglutamate synthetases from Corynebacterium species , Lactobacillus casei , Streptococcus faecalis , and Chinese hamster ovary ( CHO ) cells are described .
	manualset3
167011	3	412695	7	NULL	NULL	0	NULL	Corynebacterium species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The substrate specificities of folylpolyglutamate synthetases from Corynebacterium species , Lactobacillus casei , Streptococcus faecalis , and Chinese hamster ovary ( CHO ) cells are described .
	manualset3
167012	4	412695	7	NULL	NULL	0	NULL	 Lactobacillus casei	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The substrate specificities of folylpolyglutamate synthetases from Corynebacterium species , Lactobacillus casei , Streptococcus faecalis , and Chinese hamster ovary ( CHO ) cells are described .
	manualset3
167013	5	412695	7	NULL	NULL	0	NULL	Streptococcus faecalis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The substrate specificities of folylpolyglutamate synthetases from Corynebacterium species , Lactobacillus casei , Streptococcus faecalis , and Chinese hamster ovary ( CHO ) cells are described .
	manualset3
167014	6	412695	7	NULL	NULL	0	NULL	Chinese hamster ovary ( CHO ) cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The substrate specificities of folylpolyglutamate synthetases from Corynebacterium species , Lactobacillus casei , Streptococcus faecalis , and Chinese hamster ovary ( CHO ) cells are described .
	manualset3
167787	2	412695	7	NULL	NULL	0	NULL	folylpolyglutamate synthetases	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The substrate specificities of folylpolyglutamate synthetases from Corynebacterium species , Lactobacillus casei , Streptococcus faecalis , and Chinese hamster ovary ( CHO ) cells are described .
	manualset3
167015	1	412696	7	NULL	NULL	0	NULL	subventricular zone	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The subventricular zone : new molecular and cellular developments .
	manualset3
167016	2	412696	7	NULL	NULL	NULL	NULL	 new molecular developments	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The subventricular zone : new molecular and cellular developments .
	manualset3
167017	3	412696	7	NULL	NULL	NULL	NULL	cellular developments	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The subventricular zone : new molecular and cellular developments .
	manualset3
167018	1	412697	7	NULL	NULL	NULL	NULL	success-rate	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The success-rate ( non-transendoscopic technique 94 vs transendoscopic technique 79 % ) , early complications ( 5 vs 11 % ) , method-specific mortality ( 0.3 vs 1 % ) , in-hospital mortality ( 3.6 vs 21 % ) and late complications ( 19 vs 33 % ) are clearly in favor of the non-transendoscopic approach .
	manualset3
167019	2	412697	7	NULL	NULL	0	NULL	non-transendoscopic technique 94	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The success-rate ( non-transendoscopic technique 94 vs transendoscopic technique 79 % ) , early complications ( 5 vs 11 % ) , method-specific mortality ( 0.3 vs 1 % ) , in-hospital mortality ( 3.6 vs 21 % ) and late complications ( 19 vs 33 % ) are clearly in favor of the non-transendoscopic approach .
	manualset3
167020	3	412697	7	NULL	NULL	0	NULL	transendoscopic technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The success-rate ( non-transendoscopic technique 94 vs transendoscopic technique 79 % ) , early complications ( 5 vs 11 % ) , method-specific mortality ( 0.3 vs 1 % ) , in-hospital mortality ( 3.6 vs 21 % ) and late complications ( 19 vs 33 % ) are clearly in favor of the non-transendoscopic approach .
	manualset3
167021	4	412697	7	NULL	NULL	0	NULL	79 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The success-rate ( non-transendoscopic technique 94 vs transendoscopic technique 79 % ) , early complications ( 5 vs 11 % ) , method-specific mortality ( 0.3 vs 1 % ) , in-hospital mortality ( 3.6 vs 21 % ) and late complications ( 19 vs 33 % ) are clearly in favor of the non-transendoscopic approach .
	manualset3
167022	5	412697	7	NULL	NULL	0	NULL	early complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The success-rate ( non-transendoscopic technique 94 vs transendoscopic technique 79 % ) , early complications ( 5 vs 11 % ) , method-specific mortality ( 0.3 vs 1 % ) , in-hospital mortality ( 3.6 vs 21 % ) and late complications ( 19 vs 33 % ) are clearly in favor of the non-transendoscopic approach .
	manualset3
167023	6	412697	7	NULL	NULL	0	NULL	5 vs 11 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The success-rate ( non-transendoscopic technique 94 vs transendoscopic technique 79 % ) , early complications ( 5 vs 11 % ) , method-specific mortality ( 0.3 vs 1 % ) , in-hospital mortality ( 3.6 vs 21 % ) and late complications ( 19 vs 33 % ) are clearly in favor of the non-transendoscopic approach .
	manualset3
167024	7	412697	7	NULL	NULL	0	NULL	method-specific mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The success-rate ( non-transendoscopic technique 94 vs transendoscopic technique 79 % ) , early complications ( 5 vs 11 % ) , method-specific mortality ( 0.3 vs 1 % ) , in-hospital mortality ( 3.6 vs 21 % ) and late complications ( 19 vs 33 % ) are clearly in favor of the non-transendoscopic approach .
	manualset3
167025	8	412697	7	NULL	NULL	0	NULL	0.3 vs 1 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The success-rate ( non-transendoscopic technique 94 vs transendoscopic technique 79 % ) , early complications ( 5 vs 11 % ) , method-specific mortality ( 0.3 vs 1 % ) , in-hospital mortality ( 3.6 vs 21 % ) and late complications ( 19 vs 33 % ) are clearly in favor of the non-transendoscopic approach .
	manualset3
167026	9	412697	7	NULL	NULL	0	NULL	 in-hospital mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The success-rate ( non-transendoscopic technique 94 vs transendoscopic technique 79 % ) , early complications ( 5 vs 11 % ) , method-specific mortality ( 0.3 vs 1 % ) , in-hospital mortality ( 3.6 vs 21 % ) and late complications ( 19 vs 33 % ) are clearly in favor of the non-transendoscopic approach .
	manualset3
167027	10	412697	7	NULL	NULL	0	NULL	3.6 vs 21 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The success-rate ( non-transendoscopic technique 94 vs transendoscopic technique 79 % ) , early complications ( 5 vs 11 % ) , method-specific mortality ( 0.3 vs 1 % ) , in-hospital mortality ( 3.6 vs 21 % ) and late complications ( 19 vs 33 % ) are clearly in favor of the non-transendoscopic approach .
	manualset3
167028	11	412697	7	NULL	NULL	0	NULL	late complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The success-rate ( non-transendoscopic technique 94 vs transendoscopic technique 79 % ) , early complications ( 5 vs 11 % ) , method-specific mortality ( 0.3 vs 1 % ) , in-hospital mortality ( 3.6 vs 21 % ) and late complications ( 19 vs 33 % ) are clearly in favor of the non-transendoscopic approach .
	manualset3
167029	12	412697	7	NULL	NULL	0	NULL	19 vs 33 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The success-rate ( non-transendoscopic technique 94 vs transendoscopic technique 79 % ) , early complications ( 5 vs 11 % ) , method-specific mortality ( 0.3 vs 1 % ) , in-hospital mortality ( 3.6 vs 21 % ) and late complications ( 19 vs 33 % ) are clearly in favor of the non-transendoscopic approach .
	manualset3
167030	13	412697	7	NULL	NULL	0	NULL	non-transendoscopic approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The success-rate ( non-transendoscopic technique 94 vs transendoscopic technique 79 % ) , early complications ( 5 vs 11 % ) , method-specific mortality ( 0.3 vs 1 % ) , in-hospital mortality ( 3.6 vs 21 % ) and late complications ( 19 vs 33 % ) are clearly in favor of the non-transendoscopic approach .
	manualset3
167031	1	412698	7	NULL	NULL	0	NULL	Acetabular labrum tear	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetabular labrum tear in a 15-year-old male : diagnosis with correlative imaging .
	manualset3
167032	2	412698	7	NULL	NULL	0	NULL	15-year-old male	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetabular labrum tear in a 15-year-old male : diagnosis with correlative imaging .
	manualset3
167033	3	412698	7	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetabular labrum tear in a 15-year-old male : diagnosis with correlative imaging .
	manualset3
167034	4	412698	7	NULL	NULL	0	NULL	 correlative imaging	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetabular labrum tear in a 15-year-old male : diagnosis with correlative imaging .
	manualset3
167035	1	412699	7	NULL	NULL	0	NULL	grafting	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The successful grafting of the alternate mosquito toxicity onto the original lepidopteran Cry1Aa toxin demonstrates the possibility of designing and engineering a desired toxicity into any toxin of a common scaffold by reshaping the receptor binding region with desired specificities .
	manualset3
167037	2	412699	7	NULL	NULL	0	NULL	alternate mosquito toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The successful grafting of the alternate mosquito toxicity onto the original lepidopteran Cry1Aa toxin demonstrates the possibility of designing and engineering a desired toxicity into any toxin of a common scaffold by reshaping the receptor binding region with desired specificities .
	manualset3
167038	3	412699	7	NULL	NULL	0	NULL	 original lepidopteran Cry1Aa toxin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The successful grafting of the alternate mosquito toxicity onto the original lepidopteran Cry1Aa toxin demonstrates the possibility of designing and engineering a desired toxicity into any toxin of a common scaffold by reshaping the receptor binding region with desired specificities .
	manualset3
167039	4	412699	7	NULL	NULL	0	NULL	possibility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The successful grafting of the alternate mosquito toxicity onto the original lepidopteran Cry1Aa toxin demonstrates the possibility of designing and engineering a desired toxicity into any toxin of a common scaffold by reshaping the receptor binding region with desired specificities .
	manualset3
167040	5	412699	7	NULL	NULL	0	NULL	designing 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The successful grafting of the alternate mosquito toxicity onto the original lepidopteran Cry1Aa toxin demonstrates the possibility of designing and engineering a desired toxicity into any toxin of a common scaffold by reshaping the receptor binding region with desired specificities .
	manualset3
167041	6	412699	7	NULL	NULL	0	NULL	engineering	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The successful grafting of the alternate mosquito toxicity onto the original lepidopteran Cry1Aa toxin demonstrates the possibility of designing and engineering a desired toxicity into any toxin of a common scaffold by reshaping the receptor binding region with desired specificities .
	manualset3
167042	7	412699	7	NULL	NULL	0	NULL	desired toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The successful grafting of the alternate mosquito toxicity onto the original lepidopteran Cry1Aa toxin demonstrates the possibility of designing and engineering a desired toxicity into any toxin of a common scaffold by reshaping the receptor binding region with desired specificities .
	manualset3
167043	8	412699	7	NULL	NULL	0	NULL	toxin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The successful grafting of the alternate mosquito toxicity onto the original lepidopteran Cry1Aa toxin demonstrates the possibility of designing and engineering a desired toxicity into any toxin of a common scaffold by reshaping the receptor binding region with desired specificities .
	manualset3
167044	9	412699	7	NULL	NULL	0	NULL	common scaffold	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The successful grafting of the alternate mosquito toxicity onto the original lepidopteran Cry1Aa toxin demonstrates the possibility of designing and engineering a desired toxicity into any toxin of a common scaffold by reshaping the receptor binding region with desired specificities .
	manualset3
167045	10	412699	7	NULL	NULL	0	NULL	receptor binding region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The successful grafting of the alternate mosquito toxicity onto the original lepidopteran Cry1Aa toxin demonstrates the possibility of designing and engineering a desired toxicity into any toxin of a common scaffold by reshaping the receptor binding region with desired specificities .
	manualset3
167788	11	412699	7	NULL	NULL	0	NULL	reshaping	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The successful grafting of the alternate mosquito toxicity onto the original lepidopteran Cry1Aa toxin demonstrates the possibility of designing and engineering a desired toxicity into any toxin of a common scaffold by reshaping the receptor binding region with desired specificities .
	manualset3
169200	12	412699	7	NULL	NULL	0	NULL	specificities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The successful grafting of the alternate mosquito toxicity onto the original lepidopteran Cry1Aa toxin demonstrates the possibility of designing and engineering a desired toxicity into any toxin of a common scaffold by reshaping the receptor binding region with desired specificities .
	manualset3
167046	1	412700	7	NULL	NULL	0	NULL	sudden death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The sudden death is often the first symptom of BrS and appears most often already during the fourth decade of life of BrS patients .
	manualset3
167047	2	412700	7	NULL	NULL	0	NULL	first symptom	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The sudden death is often the first symptom of BrS and appears most often already during the fourth decade of life of BrS patients .
	manualset3
167048	3	412700	7	NULL	NULL	0	NULL	BrS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The sudden death is often the first symptom of BrS and appears most often already during the fourth decade of life of BrS patients .
	manualset3
167049	4	412700	7	NULL	NULL	0	NULL	fourth decade	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The sudden death is often the first symptom of BrS and appears most often already during the fourth decade of life of BrS patients .
	manualset3
167050	5	412700	7	NULL	NULL	0	NULL	life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The sudden death is often the first symptom of BrS and appears most often already during the fourth decade of life of BrS patients .
	manualset3
167051	6	412700	7	NULL	NULL	0	NULL	BrS patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The sudden death is often the first symptom of BrS and appears most often already during the fourth decade of life of BrS patients .
	manualset3
167052	1	412701	7	NULL	NULL	0	NULL	sudden infant death syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The sudden infant death syndrome peaks in the second and third month of life .
	manualset3
167053	2	412701	7	NULL	NULL	0	NULL	second month	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The sudden infant death syndrome peaks in the second and third month of life .
	manualset3
167054	3	412701	7	NULL	NULL	0	NULL	third month	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The sudden infant death syndrome peaks in the second and third month of life .
	manualset3
167055	4	412701	7	NULL	NULL	0	NULL	life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The sudden infant death syndrome peaks in the second and third month of life .
	manualset3
167056	1	412702	7	NULL	NULL	0	NULL	suitability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The suitability of a granulated zero valent iron ( ZVI ) permeable reactive barrier ( PRB ) remediation strategy was investigated for tribromoethene ( TriBE ) , cis-1 , 2 - dibromoethene ( c-DBE ) , trans-1 , 2 - dibromoethene ( t-DBE ) and vinyl bromide ( VB ) , via batch and large-scale column experiments that were subsequently analyzed by reactive transport modelling .
	manualset3
167057	2	412702	7	NULL	NULL	0	NULL	granulated zero valent iron ( ZVI )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The suitability of a granulated zero valent iron ( ZVI ) permeable reactive barrier ( PRB ) remediation strategy was investigated for tribromoethene ( TriBE ) , cis-1 , 2 - dibromoethene ( c-DBE ) , trans-1 , 2 - dibromoethene ( t-DBE ) and vinyl bromide ( VB ) , via batch and large-scale column experiments that were subsequently analyzed by reactive transport modelling .
	manualset3
167058	3	412702	7	NULL	NULL	0	NULL	permeable reactive barrier ( PRB ) remediation strategy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The suitability of a granulated zero valent iron ( ZVI ) permeable reactive barrier ( PRB ) remediation strategy was investigated for tribromoethene ( TriBE ) , cis-1 , 2 - dibromoethene ( c-DBE ) , trans-1 , 2 - dibromoethene ( t-DBE ) and vinyl bromide ( VB ) , via batch and large-scale column experiments that were subsequently analyzed by reactive transport modelling .
	manualset3
167059	4	412702	7	NULL	NULL	0	NULL	tribromoethene ( TriBE )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The suitability of a granulated zero valent iron ( ZVI ) permeable reactive barrier ( PRB ) remediation strategy was investigated for tribromoethene ( TriBE ) , cis-1 , 2 - dibromoethene ( c-DBE ) , trans-1 , 2 - dibromoethene ( t-DBE ) and vinyl bromide ( VB ) , via batch and large-scale column experiments that were subsequently analyzed by reactive transport modelling .
	manualset3
167060	5	412702	7	NULL	NULL	0	NULL	cis-1 , 2 - dibromoethene ( c-DBE )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The suitability of a granulated zero valent iron ( ZVI ) permeable reactive barrier ( PRB ) remediation strategy was investigated for tribromoethene ( TriBE ) , cis-1 , 2 - dibromoethene ( c-DBE ) , trans-1 , 2 - dibromoethene ( t-DBE ) and vinyl bromide ( VB ) , via batch and large-scale column experiments that were subsequently analyzed by reactive transport modelling .
	manualset3
167061	6	412702	7	NULL	NULL	0	NULL	trans-1 , 2 - dibromoethene ( t-DBE )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The suitability of a granulated zero valent iron ( ZVI ) permeable reactive barrier ( PRB ) remediation strategy was investigated for tribromoethene ( TriBE ) , cis-1 , 2 - dibromoethene ( c-DBE ) , trans-1 , 2 - dibromoethene ( t-DBE ) and vinyl bromide ( VB ) , via batch and large-scale column experiments that were subsequently analyzed by reactive transport modelling .
	manualset3
167062	7	412702	7	NULL	NULL	0	NULL	vinyl bromide ( VB )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The suitability of a granulated zero valent iron ( ZVI ) permeable reactive barrier ( PRB ) remediation strategy was investigated for tribromoethene ( TriBE ) , cis-1 , 2 - dibromoethene ( c-DBE ) , trans-1 , 2 - dibromoethene ( t-DBE ) and vinyl bromide ( VB ) , via batch and large-scale column experiments that were subsequently analyzed by reactive transport modelling .
	manualset3
167063	8	412702	7	NULL	NULL	0	NULL	batch and large-scale column experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The suitability of a granulated zero valent iron ( ZVI ) permeable reactive barrier ( PRB ) remediation strategy was investigated for tribromoethene ( TriBE ) , cis-1 , 2 - dibromoethene ( c-DBE ) , trans-1 , 2 - dibromoethene ( t-DBE ) and vinyl bromide ( VB ) , via batch and large-scale column experiments that were subsequently analyzed by reactive transport modelling .
	manualset3
167064	9	412702	7	NULL	NULL	0	NULL	 reactive transport modelling	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The suitability of a granulated zero valent iron ( ZVI ) permeable reactive barrier ( PRB ) remediation strategy was investigated for tribromoethene ( TriBE ) , cis-1 , 2 - dibromoethene ( c-DBE ) , trans-1 , 2 - dibromoethene ( t-DBE ) and vinyl bromide ( VB ) , via batch and large-scale column experiments that were subsequently analyzed by reactive transport modelling .
	manualset3
167065	1	412703	7	NULL	NULL	0	NULL	sulfhydryl characterizing agent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The sulfhydryl characterizing agent N-ethylmaleimide ( NEM ) differentially affected ( 3H ) 5-HT uptake and ( 3H ) IMI binding in human platelet preparations .
	manualset3
167066	2	412703	7	NULL	NULL	0	NULL	N-ethylmaleimide ( NEM )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The sulfhydryl characterizing agent N-ethylmaleimide ( NEM ) differentially affected ( 3H ) 5-HT uptake and ( 3H ) IMI binding in human platelet preparations .
	manualset3
167067	3	412703	7	NULL	NULL	0	NULL	( 3H ) 5-HT uptake 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The sulfhydryl characterizing agent N-ethylmaleimide ( NEM ) differentially affected ( 3H ) 5-HT uptake and ( 3H ) IMI binding in human platelet preparations .
	manualset3
167068	4	412703	7	NULL	NULL	0	NULL	( 3H ) IMI binding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The sulfhydryl characterizing agent N-ethylmaleimide ( NEM ) differentially affected ( 3H ) 5-HT uptake and ( 3H ) IMI binding in human platelet preparations .
	manualset3
167069	5	412703	7	NULL	NULL	0	NULL	human platelet preparations	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The sulfhydryl characterizing agent N-ethylmaleimide ( NEM ) differentially affected ( 3H ) 5-HT uptake and ( 3H ) IMI binding in human platelet preparations .
	manualset3
167070	1	412704	7	NULL	NULL	0	NULL	Acetate metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetate metabolism was markedly stimulated by the presence of polyglucose .
	manualset3
167071	2	412704	7	NULL	NULL	0	NULL	presence 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetate metabolism was markedly stimulated by the presence of polyglucose .
	manualset3
167072	3	412704	7	NULL	NULL	NULL	NULL	polyglucose	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Acetate metabolism was markedly stimulated by the presence of polyglucose .
	manualset3
167073	1	412705	7	NULL	NULL	0	NULL	sulfide-type modification products	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The sulfide-type modification products were stable , whereas the formation of the disulfide-type modification products was reversed by the action of endogenous SH compounds such as glutathione .
	manualset3
167074	2	412705	7	NULL	NULL	0	NULL	formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The sulfide-type modification products were stable , whereas the formation of the disulfide-type modification products was reversed by the action of endogenous SH compounds such as glutathione .
	manualset3
167075	3	412705	7	NULL	NULL	0	NULL	disulfide-type modification products	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The sulfide-type modification products were stable , whereas the formation of the disulfide-type modification products was reversed by the action of endogenous SH compounds such as glutathione .
	manualset3
167076	4	412705	7	NULL	NULL	0	NULL	action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The sulfide-type modification products were stable , whereas the formation of the disulfide-type modification products was reversed by the action of endogenous SH compounds such as glutathione .
	manualset3
167077	5	412705	7	NULL	NULL	0	NULL	endogenous SH compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The sulfide-type modification products were stable , whereas the formation of the disulfide-type modification products was reversed by the action of endogenous SH compounds such as glutathione .
	manualset3
167078	6	412705	7	NULL	NULL	0	NULL	glutathione	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The sulfide-type modification products were stable , whereas the formation of the disulfide-type modification products was reversed by the action of endogenous SH compounds such as glutathione .
	manualset3
167079	1	412706	7	NULL	NULL	0	NULL	 superior colliculus ( SC ) 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The superior colliculus ( SC ) plays a prominent role in the gap effect for saccades , and recent data indicate that this structure also plays some role in the control of pursuit .
	manualset3
167080	2	412706	7	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The superior colliculus ( SC ) plays a prominent role in the gap effect for saccades , and recent data indicate that this structure also plays some role in the control of pursuit .
	manualset3
167081	3	412706	7	NULL	NULL	0	NULL	gap effect 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The superior colliculus ( SC ) plays a prominent role in the gap effect for saccades , and recent data indicate that this structure also plays some role in the control of pursuit .
	manualset3
167082	4	412706	7	NULL	NULL	0	NULL	saccades	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The superior colliculus ( SC ) plays a prominent role in the gap effect for saccades , and recent data indicate that this structure also plays some role in the control of pursuit .
	manualset3
167083	5	412706	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The superior colliculus ( SC ) plays a prominent role in the gap effect for saccades , and recent data indicate that this structure also plays some role in the control of pursuit .
	manualset3
167084	6	412706	7	NULL	NULL	0	NULL	structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The superior colliculus ( SC ) plays a prominent role in the gap effect for saccades , and recent data indicate that this structure also plays some role in the control of pursuit .
	manualset3
167085	7	412706	7	NULL	NULL	0	NULL	role 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The superior colliculus ( SC ) plays a prominent role in the gap effect for saccades , and recent data indicate that this structure also plays some role in the control of pursuit .
	manualset3
173649	8	412706	7	NULL	NULL	0	NULL	control	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The superior colliculus ( SC ) plays a prominent role in the gap effect for saccades , and recent data indicate that this structure also plays some role in the control of pursuit .
	manualset3
173650	9	412706	7	NULL	NULL	0	NULL	pursuit 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The superior colliculus ( SC ) plays a prominent role in the gap effect for saccades , and recent data indicate that this structure also plays some role in the control of pursuit .
	manualset3
167086	1	412707	7	NULL	NULL	0	NULL	supplementation	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The supplementation of the growth medium with R. rosea extract decreased survival of exponentially growing S. cerevisiae cells under H ( 2 ) O ( 2 ) - induced oxidative stress , but increased viability and reproduction success of yeast cells in stationary phase .
	manualset3
167087	2	412707	7	NULL	NULL	0	NULL	growth medium	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The supplementation of the growth medium with R. rosea extract decreased survival of exponentially growing S. cerevisiae cells under H ( 2 ) O ( 2 ) - induced oxidative stress , but increased viability and reproduction success of yeast cells in stationary phase .
	manualset3
167088	3	412707	7	NULL	NULL	0	NULL	R. rosea extract	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The supplementation of the growth medium with R. rosea extract decreased survival of exponentially growing S. cerevisiae cells under H ( 2 ) O ( 2 ) - induced oxidative stress , but increased viability and reproduction success of yeast cells in stationary phase .
	manualset3
167089	4	412707	7	NULL	NULL	0	NULL	survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The supplementation of the growth medium with R. rosea extract decreased survival of exponentially growing S. cerevisiae cells under H ( 2 ) O ( 2 ) - induced oxidative stress , but increased viability and reproduction success of yeast cells in stationary phase .
	manualset3
167090	5	412707	7	NULL	NULL	0	NULL	S. cerevisiae cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The supplementation of the growth medium with R. rosea extract decreased survival of exponentially growing S. cerevisiae cells under H ( 2 ) O ( 2 ) - induced oxidative stress , but increased viability and reproduction success of yeast cells in stationary phase .
	manualset3
167091	6	412707	7	NULL	NULL	0	NULL	H ( 2 ) O ( 2 ) - induced oxidative stress	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The supplementation of the growth medium with R. rosea extract decreased survival of exponentially growing S. cerevisiae cells under H ( 2 ) O ( 2 ) - induced oxidative stress , but increased viability and reproduction success of yeast cells in stationary phase .
	manualset3
167092	7	412707	7	NULL	NULL	0	NULL	viability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The supplementation of the growth medium with R. rosea extract decreased survival of exponentially growing S. cerevisiae cells under H ( 2 ) O ( 2 ) - induced oxidative stress , but increased viability and reproduction success of yeast cells in stationary phase .
	manualset3
167093	8	412707	7	NULL	NULL	NULL	NULL	reproduction success	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The supplementation of the growth medium with R. rosea extract decreased survival of exponentially growing S. cerevisiae cells under H ( 2 ) O ( 2 ) - induced oxidative stress , but increased viability and reproduction success of yeast cells in stationary phase .
	manualset3
167094	9	412707	7	NULL	NULL	0	NULL	yeast cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The supplementation of the growth medium with R. rosea extract decreased survival of exponentially growing S. cerevisiae cells under H ( 2 ) O ( 2 ) - induced oxidative stress , but increased viability and reproduction success of yeast cells in stationary phase .
	manualset3
167095	10	412707	7	NULL	NULL	0	NULL	stationary phase	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The supplementation of the growth medium with R. rosea extract decreased survival of exponentially growing S. cerevisiae cells under H ( 2 ) O ( 2 ) - induced oxidative stress , but increased viability and reproduction success of yeast cells in stationary phase .
	manualset3
167096	1	412708	7	NULL	NULL	0	NULL	support	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The support of adenosine release from adenosine kinase deficient ES cells by silk substrates .
	manualset3
167097	2	412708	7	NULL	NULL	0	NULL	adenosine release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The support of adenosine release from adenosine kinase deficient ES cells by silk substrates .
	manualset3
167098	3	412708	7	NULL	NULL	0	NULL	adenosine kinase deficient ES cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The support of adenosine release from adenosine kinase deficient ES cells by silk substrates .
	manualset3
167099	4	412708	7	NULL	NULL	0	NULL	silk substrates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The support of adenosine release from adenosine kinase deficient ES cells by silk substrates .
	manualset3
167100	1	412709	7	NULL	NULL	0	NULL	supra mediocrural route	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The supra mediocrural route ) .
	manualset3
167101	1	412710	7	NULL	NULL	0	NULL	 surface	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The surface of a Petri dish provides such an environment , but a more detailed understanding of microbial growth on Petri dishes is necessary to interpret such experiments .
	manualset3
167102	2	412710	7	NULL	NULL	0	NULL	Petri dish	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The surface of a Petri dish provides such an environment , but a more detailed understanding of microbial growth on Petri dishes is necessary to interpret such experiments .
	manualset3
167103	3	412710	7	NULL	NULL	0	NULL	environment	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The surface of a Petri dish provides such an environment , but a more detailed understanding of microbial growth on Petri dishes is necessary to interpret such experiments .
	manualset3
167104	4	412710	7	NULL	NULL	NULL	NULL	understanding	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The surface of a Petri dish provides such an environment , but a more detailed understanding of microbial growth on Petri dishes is necessary to interpret such experiments .
	manualset3
167105	5	412710	7	NULL	NULL	0	NULL	microbial growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The surface of a Petri dish provides such an environment , but a more detailed understanding of microbial growth on Petri dishes is necessary to interpret such experiments .
	manualset3
167106	6	412710	7	NULL	NULL	0	NULL	Petri dishes	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The surface of a Petri dish provides such an environment , but a more detailed understanding of microbial growth on Petri dishes is necessary to interpret such experiments .
	manualset3
167107	7	412710	7	NULL	NULL	0	NULL	experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The surface of a Petri dish provides such an environment , but a more detailed understanding of microbial growth on Petri dishes is necessary to interpret such experiments .
	manualset3
167108	1	412711	7	NULL	NULL	NULL	NULL	Acetazolamide 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Acetazolamide ( 50 mumols/l ) , a potent inhibitor of carbonic anhydrase mainly present in the MRC , reduced selectively by 31 % O2 uptake of the MRC-rich epithelia ( NaNO3 acclimated ) .
	manualset3
167109	2	412711	7	NULL	NULL	0	NULL	inhibitor 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetazolamide ( 50 mumols/l ) , a potent inhibitor of carbonic anhydrase mainly present in the MRC , reduced selectively by 31 % O2 uptake of the MRC-rich epithelia ( NaNO3 acclimated ) .
	manualset3
167110	3	412711	7	NULL	NULL	0	NULL	carbonic anhydrase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetazolamide ( 50 mumols/l ) , a potent inhibitor of carbonic anhydrase mainly present in the MRC , reduced selectively by 31 % O2 uptake of the MRC-rich epithelia ( NaNO3 acclimated ) .
	manualset3
167111	4	412711	7	NULL	NULL	0	NULL	MRC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetazolamide ( 50 mumols/l ) , a potent inhibitor of carbonic anhydrase mainly present in the MRC , reduced selectively by 31 % O2 uptake of the MRC-rich epithelia ( NaNO3 acclimated ) .
	manualset3
167112	5	412711	7	NULL	NULL	0	NULL	 31 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetazolamide ( 50 mumols/l ) , a potent inhibitor of carbonic anhydrase mainly present in the MRC , reduced selectively by 31 % O2 uptake of the MRC-rich epithelia ( NaNO3 acclimated ) .
	manualset3
167113	6	412711	7	NULL	NULL	0	NULL	O2 uptake	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetazolamide ( 50 mumols/l ) , a potent inhibitor of carbonic anhydrase mainly present in the MRC , reduced selectively by 31 % O2 uptake of the MRC-rich epithelia ( NaNO3 acclimated ) .
	manualset3
167114	7	412711	7	NULL	NULL	0	NULL	MRC-rich epithelia	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetazolamide ( 50 mumols/l ) , a potent inhibitor of carbonic anhydrase mainly present in the MRC , reduced selectively by 31 % O2 uptake of the MRC-rich epithelia ( NaNO3 acclimated ) .
	manualset3
167115	8	412711	7	NULL	NULL	0	NULL	NaNO3	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetazolamide ( 50 mumols/l ) , a potent inhibitor of carbonic anhydrase mainly present in the MRC , reduced selectively by 31 % O2 uptake of the MRC-rich epithelia ( NaNO3 acclimated ) .
	manualset3
167789	9	412711	7	NULL	NULL	0	NULL	50 mumols/l 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetazolamide ( 50 mumols/l ) , a potent inhibitor of carbonic anhydrase mainly present in the MRC , reduced selectively by 31 % O2 uptake of the MRC-rich epithelia ( NaNO3 acclimated ) .
	manualset3
167116	1	412712	7	NULL	NULL	0	NULL	surface	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The surface of the prosthesis is unlike other uncemented prostheses since the rough surface is formed by multiple 1-mm diameter beads that are cast as an integral part of the prosthesis and increase its surface area four times .
	manualset3
167117	2	412712	7	NULL	NULL	0	NULL	prosthesis	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The surface of the prosthesis is unlike other uncemented prostheses since the rough surface is formed by multiple 1-mm diameter beads that are cast as an integral part of the prosthesis and increase its surface area four times .
	manualset3
167118	3	412712	7	NULL	NULL	0	NULL	uncemented prostheses	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The surface of the prosthesis is unlike other uncemented prostheses since the rough surface is formed by multiple 1-mm diameter beads that are cast as an integral part of the prosthesis and increase its surface area four times .
	manualset3
167119	4	412712	7	NULL	NULL	0	NULL	rough surface	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The surface of the prosthesis is unlike other uncemented prostheses since the rough surface is formed by multiple 1-mm diameter beads that are cast as an integral part of the prosthesis and increase its surface area four times .
	manualset3
167120	5	412712	7	NULL	NULL	0	NULL	1-mm diameter	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The surface of the prosthesis is unlike other uncemented prostheses since the rough surface is formed by multiple 1-mm diameter beads that are cast as an integral part of the prosthesis and increase its surface area four times .
	manualset3
167121	6	412712	7	NULL	NULL	0	NULL	beads	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The surface of the prosthesis is unlike other uncemented prostheses since the rough surface is formed by multiple 1-mm diameter beads that are cast as an integral part of the prosthesis and increase its surface area four times .
	manualset3
167122	7	412712	7	NULL	NULL	0	NULL	 integral part 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The surface of the prosthesis is unlike other uncemented prostheses since the rough surface is formed by multiple 1-mm diameter beads that are cast as an integral part of the prosthesis and increase its surface area four times .
	manualset3
167123	8	412712	7	NULL	NULL	0	NULL	prosthesis 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The surface of the prosthesis is unlike other uncemented prostheses since the rough surface is formed by multiple 1-mm diameter beads that are cast as an integral part of the prosthesis and increase its surface area four times .
	manualset3
167124	9	412712	7	NULL	NULL	0	NULL	 surface area	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The surface of the prosthesis is unlike other uncemented prostheses since the rough surface is formed by multiple 1-mm diameter beads that are cast as an integral part of the prosthesis and increase its surface area four times .
	manualset3
167125	10	412712	7	NULL	NULL	NULL	NULL	four times	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The surface of the prosthesis is unlike other uncemented prostheses since the rough surface is formed by multiple 1-mm diameter beads that are cast as an integral part of the prosthesis and increase its surface area four times .
	manualset3
167126	1	412713	7	NULL	NULL	0	NULL	surgical approach	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The surgical approach in a patient with a ventriculoperitoneal shunt in need of abdominal surgery remains controversial .
	manualset3
167127	2	412713	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The surgical approach in a patient with a ventriculoperitoneal shunt in need of abdominal surgery remains controversial .
	manualset3
167128	3	412713	7	NULL	NULL	0	NULL	ventriculoperitoneal shunt	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The surgical approach in a patient with a ventriculoperitoneal shunt in need of abdominal surgery remains controversial .
	manualset3
167129	4	412713	7	NULL	NULL	0	NULL	abdominal surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The surgical approach in a patient with a ventriculoperitoneal shunt in need of abdominal surgery remains controversial .
	manualset3
167130	1	412714	7	NULL	NULL	0	NULL	surgical experience	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The surgical experience of a decade of acoustic tumor surgery is discussed .
	manualset3
167131	2	412714	7	NULL	NULL	0	NULL	decade	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The surgical experience of a decade of acoustic tumor surgery is discussed .
	manualset3
167132	3	412714	7	NULL	NULL	0	NULL	acoustic tumor surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The surgical experience of a decade of acoustic tumor surgery is discussed .
	manualset3
167133	1	412715	7	NULL	NULL	0	NULL	surgical technique	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The surgical technique must be strict .
	manualset3
167134	1	412716	7	NULL	NULL	0	NULL	survey 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The survey provided valuable information on the factors that favor transmission , the clinical signs , the importance of relapses and the therapies used .
	manualset3
167135	2	412716	7	NULL	NULL	0	NULL	information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The survey provided valuable information on the factors that favor transmission , the clinical signs , the importance of relapses and the therapies used .
	manualset3
167136	3	412716	7	NULL	NULL	0	NULL	factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The survey provided valuable information on the factors that favor transmission , the clinical signs , the importance of relapses and the therapies used .
	manualset3
167137	4	412716	7	NULL	NULL	0	NULL	transmission	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The survey provided valuable information on the factors that favor transmission , the clinical signs , the importance of relapses and the therapies used .
	manualset3
167138	5	412716	7	NULL	NULL	0	NULL	clinical signs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The survey provided valuable information on the factors that favor transmission , the clinical signs , the importance of relapses and the therapies used .
	manualset3
167139	6	412716	7	NULL	NULL	0	NULL	relapses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The survey provided valuable information on the factors that favor transmission , the clinical signs , the importance of relapses and the therapies used .
	manualset3
167140	7	412716	7	NULL	NULL	0	NULL	therapies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The survey provided valuable information on the factors that favor transmission , the clinical signs , the importance of relapses and the therapies used .
	manualset3
167141	1	412717	7	NULL	NULL	0	NULL	survey return rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The survey return rate was 100 % ( 28/28 ) .
	manualset3
167142	2	412717	7	NULL	NULL	0	NULL	100 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The survey return rate was 100 % ( 28/28 ) .
	manualset3
167143	3	412717	7	NULL	NULL	0	NULL	28/28	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The survey return rate was 100 % ( 28/28 ) .
	manualset3
167144	1	412718	7	NULL	NULL	0	NULL	survival rates 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The survival rates of the Day-9 embryos based on reappearance of blastocoele , expansion , and hatching after 48 h of post-thaw culture were significantly lower ( P & lt ; 0.01 ) than those of the Day-7 and 8 embryos , in all of the cryoprotectants tested .
	manualset3
167145	2	412718	7	NULL	NULL	0	NULL	Day-9 embryos	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The survival rates of the Day-9 embryos based on reappearance of blastocoele , expansion , and hatching after 48 h of post-thaw culture were significantly lower ( P & lt ; 0.01 ) than those of the Day-7 and 8 embryos , in all of the cryoprotectants tested .
	manualset3
167146	3	412718	7	NULL	NULL	0	NULL	blastocoele	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The survival rates of the Day-9 embryos based on reappearance of blastocoele , expansion , and hatching after 48 h of post-thaw culture were significantly lower ( P & lt ; 0.01 ) than those of the Day-7 and 8 embryos , in all of the cryoprotectants tested .
	manualset3
167147	4	412718	7	NULL	NULL	0	NULL	 expansion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The survival rates of the Day-9 embryos based on reappearance of blastocoele , expansion , and hatching after 48 h of post-thaw culture were significantly lower ( P & lt ; 0.01 ) than those of the Day-7 and 8 embryos , in all of the cryoprotectants tested .
	manualset3
167148	5	412718	7	NULL	NULL	0	NULL	hatching 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The survival rates of the Day-9 embryos based on reappearance of blastocoele , expansion , and hatching after 48 h of post-thaw culture were significantly lower ( P & lt ; 0.01 ) than those of the Day-7 and 8 embryos , in all of the cryoprotectants tested .
	manualset3
167149	6	412718	7	NULL	NULL	0	NULL	48 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The survival rates of the Day-9 embryos based on reappearance of blastocoele , expansion , and hatching after 48 h of post-thaw culture were significantly lower ( P & lt ; 0.01 ) than those of the Day-7 and 8 embryos , in all of the cryoprotectants tested .
	manualset3
167150	7	412718	7	NULL	NULL	0	NULL	post-thaw culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The survival rates of the Day-9 embryos based on reappearance of blastocoele , expansion , and hatching after 48 h of post-thaw culture were significantly lower ( P & lt ; 0.01 ) than those of the Day-7 and 8 embryos , in all of the cryoprotectants tested .
	manualset3
167151	8	412718	7	NULL	NULL	0	NULL	P & lt ; 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The survival rates of the Day-9 embryos based on reappearance of blastocoele , expansion , and hatching after 48 h of post-thaw culture were significantly lower ( P & lt ; 0.01 ) than those of the Day-7 and 8 embryos , in all of the cryoprotectants tested .
	manualset3
167152	9	412718	7	NULL	NULL	0	NULL	Day-7 embryos	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The survival rates of the Day-9 embryos based on reappearance of blastocoele , expansion , and hatching after 48 h of post-thaw culture were significantly lower ( P & lt ; 0.01 ) than those of the Day-7 and 8 embryos , in all of the cryoprotectants tested .
	manualset3
167153	10	412718	7	NULL	NULL	0	NULL	Day-8 embryos	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The survival rates of the Day-9 embryos based on reappearance of blastocoele , expansion , and hatching after 48 h of post-thaw culture were significantly lower ( P & lt ; 0.01 ) than those of the Day-7 and 8 embryos , in all of the cryoprotectants tested .
	manualset3
167154	11	412718	7	NULL	NULL	0	NULL	cryoprotectants	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The survival rates of the Day-9 embryos based on reappearance of blastocoele , expansion , and hatching after 48 h of post-thaw culture were significantly lower ( P & lt ; 0.01 ) than those of the Day-7 and 8 embryos , in all of the cryoprotectants tested .
	manualset3
167155	1	412719	7	NULL	NULL	0	NULL	suspected diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The suspected diagnosis was thus brucellosis taking the typical anamnesis into account .
	manualset3
167156	2	412719	7	NULL	NULL	0	NULL	brucellosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The suspected diagnosis was thus brucellosis taking the typical anamnesis into account .
	manualset3
167157	3	412719	7	NULL	NULL	NULL	NULL	anamnesis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The suspected diagnosis was thus brucellosis taking the typical anamnesis into account .
	manualset3
167158	1	412720	7	NULL	NULL	0	NULL	 swelling laws	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The swelling laws , derived from the interparticle distances obtained by SAXS , display a transition from isotropic swelling at low volume fractions to lamellar swelling at higher volume fractions .
	manualset3
167159	2	412720	7	NULL	NULL	0	NULL	interparticle distances	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The swelling laws , derived from the interparticle distances obtained by SAXS , display a transition from isotropic swelling at low volume fractions to lamellar swelling at higher volume fractions .
	manualset3
167160	3	412720	7	NULL	NULL	0	NULL	SAXS	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The swelling laws , derived from the interparticle distances obtained by SAXS , display a transition from isotropic swelling at low volume fractions to lamellar swelling at higher volume fractions .
	manualset3
167161	4	412720	7	NULL	NULL	0	NULL	transition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The swelling laws , derived from the interparticle distances obtained by SAXS , display a transition from isotropic swelling at low volume fractions to lamellar swelling at higher volume fractions .
	manualset3
167162	5	412720	7	NULL	NULL	0	NULL	isotropic swelling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The swelling laws , derived from the interparticle distances obtained by SAXS , display a transition from isotropic swelling at low volume fractions to lamellar swelling at higher volume fractions .
	manualset3
167163	6	412720	7	NULL	NULL	0	NULL	low volume fractions	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The swelling laws , derived from the interparticle distances obtained by SAXS , display a transition from isotropic swelling at low volume fractions to lamellar swelling at higher volume fractions .
	manualset3
167164	7	412720	7	NULL	NULL	0	NULL	lamellar swelling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The swelling laws , derived from the interparticle distances obtained by SAXS , display a transition from isotropic swelling at low volume fractions to lamellar swelling at higher volume fractions .
	manualset3
167165	8	412720	7	NULL	NULL	0	NULL	higher volume fractions	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The swelling laws , derived from the interparticle distances obtained by SAXS , display a transition from isotropic swelling at low volume fractions to lamellar swelling at higher volume fractions .
	manualset3
167166	1	412721	7	NULL	NULL	0	NULL	immuno-proteasome	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The switch to an immuno-proteasome in peripheral blood mononuclear cells of patients with IgA nephropathy suggests an increased efficiency of antigen processing and presentation .
	manualset3
167167	2	412721	7	NULL	NULL	0	NULL	peripheral blood mononuclear cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The switch to an immuno-proteasome in peripheral blood mononuclear cells of patients with IgA nephropathy suggests an increased efficiency of antigen processing and presentation .
	manualset3
167168	3	412721	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The switch to an immuno-proteasome in peripheral blood mononuclear cells of patients with IgA nephropathy suggests an increased efficiency of antigen processing and presentation .
	manualset3
167169	4	412721	7	NULL	NULL	0	NULL	IgA nephropathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The switch to an immuno-proteasome in peripheral blood mononuclear cells of patients with IgA nephropathy suggests an increased efficiency of antigen processing and presentation .
	manualset3
167170	5	412721	7	NULL	NULL	0	NULL	 increased efficiency	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The switch to an immuno-proteasome in peripheral blood mononuclear cells of patients with IgA nephropathy suggests an increased efficiency of antigen processing and presentation .
	manualset3
167171	6	412721	7	NULL	NULL	0	NULL	antigen processing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The switch to an immuno-proteasome in peripheral blood mononuclear cells of patients with IgA nephropathy suggests an increased efficiency of antigen processing and presentation .
	manualset3
167172	7	412721	7	NULL	NULL	0	NULL	antigen presentation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The switch to an immuno-proteasome in peripheral blood mononuclear cells of patients with IgA nephropathy suggests an increased efficiency of antigen processing and presentation .
	manualset3
167790	8	412721	7	NULL	NULL	0	NULL	switch	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The switch to an immuno-proteasome in peripheral blood mononuclear cells of patients with IgA nephropathy suggests an increased efficiency of antigen processing and presentation .
	manualset3
167173	1	412722	7	NULL	NULL	0	NULL	switching operation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The switching operation can be implemented reproducibly with applied gas flow rates between 17 and 58 L min ( -1 ) and rotational frequencies between 400 rpm ( 6.6 Hz ) and 1200 rpm ( 20 Hz ) .
	manualset3
167174	2	412722	7	NULL	NULL	0	NULL	applied gas flow rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The switching operation can be implemented reproducibly with applied gas flow rates between 17 and 58 L min ( -1 ) and rotational frequencies between 400 rpm ( 6.6 Hz ) and 1200 rpm ( 20 Hz ) .
	manualset3
167175	3	412722	7	NULL	NULL	0	NULL	17 and 58 L min ( -1 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The switching operation can be implemented reproducibly with applied gas flow rates between 17 and 58 L min ( -1 ) and rotational frequencies between 400 rpm ( 6.6 Hz ) and 1200 rpm ( 20 Hz ) .
	manualset3
167176	4	412722	7	NULL	NULL	0	NULL	rotational frequencies	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The switching operation can be implemented reproducibly with applied gas flow rates between 17 and 58 L min ( -1 ) and rotational frequencies between 400 rpm ( 6.6 Hz ) and 1200 rpm ( 20 Hz ) .
	manualset3
167177	5	412722	7	NULL	NULL	0	NULL	400 rpm ( 6.6 Hz )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The switching operation can be implemented reproducibly with applied gas flow rates between 17 and 58 L min ( -1 ) and rotational frequencies between 400 rpm ( 6.6 Hz ) and 1200 rpm ( 20 Hz ) .
	manualset3
167178	6	412722	7	NULL	NULL	0	NULL	1200 rpm ( 20 Hz )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The switching operation can be implemented reproducibly with applied gas flow rates between 17 and 58 L min ( -1 ) and rotational frequencies between 400 rpm ( 6.6 Hz ) and 1200 rpm ( 20 Hz ) .
	manualset3
167179	1	412723	7	NULL	NULL	0	NULL	 sympathoadrenal system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The sympathoadrenal system , obesity and hypertension : an overview .
	manualset3
167180	2	412723	7	NULL	NULL	0	NULL	 obesity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The sympathoadrenal system , obesity and hypertension : an overview .
	manualset3
167181	3	412723	7	NULL	NULL	0	NULL	hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The sympathoadrenal system , obesity and hypertension : an overview .
	manualset3
167182	4	412723	7	NULL	NULL	0	NULL	 overview	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The sympathoadrenal system , obesity and hypertension : an overview .
	manualset3
167183	1	412724	7	NULL	NULL	0	NULL	 synergistic effect 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The synergistic effect of meropenem and ciprofloxacin in combination was found to be 22 % at 0.5 x the MIC and 61 % at 1 x the MIC in P. aeruginosa strains .
	manualset3
167184	2	412724	7	NULL	NULL	0	NULL	meropenem	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The synergistic effect of meropenem and ciprofloxacin in combination was found to be 22 % at 0.5 x the MIC and 61 % at 1 x the MIC in P. aeruginosa strains .
	manualset3
167185	3	412724	7	NULL	NULL	0	NULL	ciprofloxacin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The synergistic effect of meropenem and ciprofloxacin in combination was found to be 22 % at 0.5 x the MIC and 61 % at 1 x the MIC in P. aeruginosa strains .
	manualset3
167186	4	412724	7	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The synergistic effect of meropenem and ciprofloxacin in combination was found to be 22 % at 0.5 x the MIC and 61 % at 1 x the MIC in P. aeruginosa strains .
	manualset3
167187	5	412724	7	NULL	NULL	0	NULL	22 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The synergistic effect of meropenem and ciprofloxacin in combination was found to be 22 % at 0.5 x the MIC and 61 % at 1 x the MIC in P. aeruginosa strains .
	manualset3
167188	6	412724	7	NULL	NULL	0	NULL	0.5 x the MIC	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The synergistic effect of meropenem and ciprofloxacin in combination was found to be 22 % at 0.5 x the MIC and 61 % at 1 x the MIC in P. aeruginosa strains .
	manualset3
167189	7	412724	7	NULL	NULL	0	NULL	61 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The synergistic effect of meropenem and ciprofloxacin in combination was found to be 22 % at 0.5 x the MIC and 61 % at 1 x the MIC in P. aeruginosa strains .
	manualset3
167190	8	412724	7	NULL	NULL	0	NULL	1 x the MIC	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The synergistic effect of meropenem and ciprofloxacin in combination was found to be 22 % at 0.5 x the MIC and 61 % at 1 x the MIC in P. aeruginosa strains .
	manualset3
167191	9	412724	7	NULL	NULL	0	NULL	P. aeruginosa strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The synergistic effect of meropenem and ciprofloxacin in combination was found to be 22 % at 0.5 x the MIC and 61 % at 1 x the MIC in P. aeruginosa strains .
	manualset3
167192	1	412725	7	NULL	NULL	0	NULL	syngamy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The syngamy between an accidentally activated sperm nucleus with a male pronucleus-like structure and nucleus of a blastomere of gynogenetically developing clonal diploid embryo might produce a diploid-triploid mosaic individual .
	manualset3
167193	2	412725	7	NULL	NULL	0	NULL	activated sperm nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The syngamy between an accidentally activated sperm nucleus with a male pronucleus-like structure and nucleus of a blastomere of gynogenetically developing clonal diploid embryo might produce a diploid-triploid mosaic individual .
	manualset3
167194	3	412725	7	NULL	NULL	0	NULL	male pronucleus-like structure	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The syngamy between an accidentally activated sperm nucleus with a male pronucleus-like structure and nucleus of a blastomere of gynogenetically developing clonal diploid embryo might produce a diploid-triploid mosaic individual .
	manualset3
167195	4	412725	7	NULL	NULL	0	NULL	nucleus of a blastomere	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The syngamy between an accidentally activated sperm nucleus with a male pronucleus-like structure and nucleus of a blastomere of gynogenetically developing clonal diploid embryo might produce a diploid-triploid mosaic individual .
	manualset3
167196	5	412725	7	NULL	NULL	0	NULL	clonal diploid embryo	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The syngamy between an accidentally activated sperm nucleus with a male pronucleus-like structure and nucleus of a blastomere of gynogenetically developing clonal diploid embryo might produce a diploid-triploid mosaic individual .
	manualset3
167197	6	412725	7	NULL	NULL	0	NULL	diploid-triploid mosaic individual	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The syngamy between an accidentally activated sperm nucleus with a male pronucleus-like structure and nucleus of a blastomere of gynogenetically developing clonal diploid embryo might produce a diploid-triploid mosaic individual .
	manualset3
167198	1	412726	7	NULL	NULL	0	NULL	synthesis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis and characterization of nanophase hydroxyapatite using a novel dispersant-aided precipitation method .
	manualset3
167199	2	412726	7	NULL	NULL	0	NULL	characterization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis and characterization of nanophase hydroxyapatite using a novel dispersant-aided precipitation method .
	manualset3
167200	3	412726	7	NULL	NULL	0	NULL	nanophase hydroxyapatite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis and characterization of nanophase hydroxyapatite using a novel dispersant-aided precipitation method .
	manualset3
167201	4	412726	7	NULL	NULL	0	NULL	novel dispersant-aided precipitation method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis and characterization of nanophase hydroxyapatite using a novel dispersant-aided precipitation method .
	manualset3
167202	1	412727	7	NULL	NULL	0	NULL	Acetazolamide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetazolamide decreased lactate-induced alkalinisation of blood ( pH after lactate + acetazolamide 7.42 + / - 0.02 ) , but did not prevent the drop in PO2 .
	manualset3
167203	2	412727	7	NULL	NULL	0	NULL	lactate-induced alkalinisation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetazolamide decreased lactate-induced alkalinisation of blood ( pH after lactate + acetazolamide 7.42 + / - 0.02 ) , but did not prevent the drop in PO2 .
	manualset3
167204	3	412727	7	NULL	NULL	0	NULL	blood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetazolamide decreased lactate-induced alkalinisation of blood ( pH after lactate + acetazolamide 7.42 + / - 0.02 ) , but did not prevent the drop in PO2 .
	manualset3
167205	4	412727	7	NULL	NULL	0	NULL	pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetazolamide decreased lactate-induced alkalinisation of blood ( pH after lactate + acetazolamide 7.42 + / - 0.02 ) , but did not prevent the drop in PO2 .
	manualset3
167206	5	412727	7	NULL	NULL	0	NULL	lactate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetazolamide decreased lactate-induced alkalinisation of blood ( pH after lactate + acetazolamide 7.42 + / - 0.02 ) , but did not prevent the drop in PO2 .
	manualset3
167207	6	412727	7	NULL	NULL	0	NULL	acetazolamide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetazolamide decreased lactate-induced alkalinisation of blood ( pH after lactate + acetazolamide 7.42 + / - 0.02 ) , but did not prevent the drop in PO2 .
	manualset3
167208	7	412727	7	NULL	NULL	0	NULL	7.42 + / - 0.02	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetazolamide decreased lactate-induced alkalinisation of blood ( pH after lactate + acetazolamide 7.42 + / - 0.02 ) , but did not prevent the drop in PO2 .
	manualset3
167209	8	412727	7	NULL	NULL	NULL	NULL	drop in PO2	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Acetazolamide decreased lactate-induced alkalinisation of blood ( pH after lactate + acetazolamide 7.42 + / - 0.02 ) , but did not prevent the drop in PO2 .
	manualset3
167211	1	412728	7	NULL	NULL	0	NULL	synthesis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis and examination of a systematic series of 5-substituted 2-keto oxazoles as inhibitors of fatty acid amide hydrolase ( FAAH ) defined a fundamental substituent effect that led to the discovery of inhibitors with Ki 's as low as 400 pM .
	manualset3
167212	2	412728	7	NULL	NULL	0	NULL	examination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis and examination of a systematic series of 5-substituted 2-keto oxazoles as inhibitors of fatty acid amide hydrolase ( FAAH ) defined a fundamental substituent effect that led to the discovery of inhibitors with Ki 's as low as 400 pM .
	manualset3
167213	3	412728	7	NULL	NULL	NULL	NULL	systematic series	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The synthesis and examination of a systematic series of 5-substituted 2-keto oxazoles as inhibitors of fatty acid amide hydrolase ( FAAH ) defined a fundamental substituent effect that led to the discovery of inhibitors with Ki 's as low as 400 pM .
	manualset3
167214	4	412728	7	NULL	NULL	0	NULL	5-substituted 2-keto oxazoles	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis and examination of a systematic series of 5-substituted 2-keto oxazoles as inhibitors of fatty acid amide hydrolase ( FAAH ) defined a fundamental substituent effect that led to the discovery of inhibitors with Ki 's as low as 400 pM .
	manualset3
167215	5	412728	7	NULL	NULL	0	NULL	inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis and examination of a systematic series of 5-substituted 2-keto oxazoles as inhibitors of fatty acid amide hydrolase ( FAAH ) defined a fundamental substituent effect that led to the discovery of inhibitors with Ki 's as low as 400 pM .
	manualset3
167216	6	412728	7	NULL	NULL	0	NULL	fatty acid amide hydrolase ( FAAH )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis and examination of a systematic series of 5-substituted 2-keto oxazoles as inhibitors of fatty acid amide hydrolase ( FAAH ) defined a fundamental substituent effect that led to the discovery of inhibitors with Ki 's as low as 400 pM .
	manualset3
167217	7	412728	7	NULL	NULL	0	NULL	discovery	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis and examination of a systematic series of 5-substituted 2-keto oxazoles as inhibitors of fatty acid amide hydrolase ( FAAH ) defined a fundamental substituent effect that led to the discovery of inhibitors with Ki 's as low as 400 pM .
	manualset3
167218	8	412728	7	NULL	NULL	0	NULL	inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis and examination of a systematic series of 5-substituted 2-keto oxazoles as inhibitors of fatty acid amide hydrolase ( FAAH ) defined a fundamental substituent effect that led to the discovery of inhibitors with Ki 's as low as 400 pM .
	manualset3
167219	9	412728	7	NULL	NULL	0	NULL	Ki 's	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis and examination of a systematic series of 5-substituted 2-keto oxazoles as inhibitors of fatty acid amide hydrolase ( FAAH ) defined a fundamental substituent effect that led to the discovery of inhibitors with Ki 's as low as 400 pM .
	manualset3
167220	10	412728	7	NULL	NULL	0	NULL	400 pM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis and examination of a systematic series of 5-substituted 2-keto oxazoles as inhibitors of fatty acid amide hydrolase ( FAAH ) defined a fundamental substituent effect that led to the discovery of inhibitors with Ki 's as low as 400 pM .
	manualset3
167221	11	412728	7	NULL	NULL	0	NULL	substituent effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis and examination of a systematic series of 5-substituted 2-keto oxazoles as inhibitors of fatty acid amide hydrolase ( FAAH ) defined a fundamental substituent effect that led to the discovery of inhibitors with Ki 's as low as 400 pM .
	manualset3
167222	1	412729	7	NULL	NULL	0	NULL	synthesis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis of a 5 ' - O-BzH-2 ' - O - ACE-protected pseudouridine phosphoramidite is reported ( BzH , benzhydryloxy-bis ( trimethylsilyloxy ) silyl ; ACE , bis ( 2-acetoxyethoxy ) methyl ) .
	manualset3
167223	2	412729	7	NULL	NULL	0	NULL	5 ' - O-BzH-2 ' - O - ACE-protected pseudouridine phosphoramidite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis of a 5 ' - O-BzH-2 ' - O - ACE-protected pseudouridine phosphoramidite is reported ( BzH , benzhydryloxy-bis ( trimethylsilyloxy ) silyl ; ACE , bis ( 2-acetoxyethoxy ) methyl ) .
	manualset3
167224	3	412729	7	NULL	NULL	0	NULL	BzH , benzhydryloxy-bis ( trimethylsilyloxy ) silyl ; ACE , bis ( 2-acetoxyethoxy ) methyl 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis of a 5 ' - O-BzH-2 ' - O - ACE-protected pseudouridine phosphoramidite is reported ( BzH , benzhydryloxy-bis ( trimethylsilyloxy ) silyl ; ACE , bis ( 2-acetoxyethoxy ) methyl ) .
	manualset3
167225	1	412730	7	NULL	NULL	0	NULL	synthesis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis of several pyrrolidine inhibitor analogs is described that possess nanomolar in vitro potencies against the neuraminidase enzymes expressed by the B/Memphis/3 / 89 and A/N1/PR / 8/34 influenza strains .
	manualset3
167226	2	412730	7	NULL	NULL	0	NULL	pyrrolidine inhibitor analogs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis of several pyrrolidine inhibitor analogs is described that possess nanomolar in vitro potencies against the neuraminidase enzymes expressed by the B/Memphis/3 / 89 and A/N1/PR / 8/34 influenza strains .
	manualset3
167227	3	412730	7	NULL	NULL	0	NULL	nanomolar in vitro potencies	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis of several pyrrolidine inhibitor analogs is described that possess nanomolar in vitro potencies against the neuraminidase enzymes expressed by the B/Memphis/3 / 89 and A/N1/PR / 8/34 influenza strains .
	manualset3
167228	4	412730	7	NULL	NULL	0	NULL	neuraminidase enzymes	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis of several pyrrolidine inhibitor analogs is described that possess nanomolar in vitro potencies against the neuraminidase enzymes expressed by the B/Memphis/3 / 89 and A/N1/PR / 8/34 influenza strains .
	manualset3
167229	5	412730	7	NULL	NULL	0	NULL	B/Memphis/3 / 89 influenza strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis of several pyrrolidine inhibitor analogs is described that possess nanomolar in vitro potencies against the neuraminidase enzymes expressed by the B/Memphis/3 / 89 and A/N1/PR / 8/34 influenza strains .
	manualset3
167230	6	412730	7	NULL	NULL	0	NULL	A/N1/PR / 8/34 influenza strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis of several pyrrolidine inhibitor analogs is described that possess nanomolar in vitro potencies against the neuraminidase enzymes expressed by the B/Memphis/3 / 89 and A/N1/PR / 8/34 influenza strains .
	manualset3
167234	1	412731	7	NULL	NULL	0	NULL	synthetic reactions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthetic reactions and spectroscopic studied of molybdenum ( tungsten ) - copper ( silver , iron ) - sulphur ( selenium ) cluster compounds , which can be prepared by the stepwise or unit construction reactions through the successive addition ML ( L = Cl , Br , Sr , R2 etc ) across six edges or four faces of ME4 ( M = Mo , W ; E = S , Se ) tetrahedra , are described .
	manualset3
167235	2	412731	7	NULL	NULL	0	NULL	molybdenum ( tungsten ) - copper ( silver , iron ) - sulphur ( selenium ) cluster compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthetic reactions and spectroscopic studied of molybdenum ( tungsten ) - copper ( silver , iron ) - sulphur ( selenium ) cluster compounds , which can be prepared by the stepwise or unit construction reactions through the successive addition ML ( L = Cl , Br , Sr , R2 etc ) across six edges or four faces of ME4 ( M = Mo , W ; E = S , Se ) tetrahedra , are described .
	manualset3
167236	3	412731	7	NULL	NULL	0	NULL	stepwise or unit construction reactions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthetic reactions and spectroscopic studied of molybdenum ( tungsten ) - copper ( silver , iron ) - sulphur ( selenium ) cluster compounds , which can be prepared by the stepwise or unit construction reactions through the successive addition ML ( L = Cl , Br , Sr , R2 etc ) across six edges or four faces of ME4 ( M = Mo , W ; E = S , Se ) tetrahedra , are described .
	manualset3
167237	4	412731	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthetic reactions and spectroscopic studied of molybdenum ( tungsten ) - copper ( silver , iron ) - sulphur ( selenium ) cluster compounds , which can be prepared by the stepwise or unit construction reactions through the successive addition ML ( L = Cl , Br , Sr , R2 etc ) across six edges or four faces of ME4 ( M = Mo , W ; E = S , Se ) tetrahedra , are described .
	manualset3
167238	5	412731	7	NULL	NULL	0	NULL	ML ( L = Cl , Br , Sr , R2 etc ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthetic reactions and spectroscopic studied of molybdenum ( tungsten ) - copper ( silver , iron ) - sulphur ( selenium ) cluster compounds , which can be prepared by the stepwise or unit construction reactions through the successive addition ML ( L = Cl , Br , Sr , R2 etc ) across six edges or four faces of ME4 ( M = Mo , W ; E = S , Se ) tetrahedra , are described .
	manualset3
167239	6	412731	7	NULL	NULL	0	NULL	 six edges 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthetic reactions and spectroscopic studied of molybdenum ( tungsten ) - copper ( silver , iron ) - sulphur ( selenium ) cluster compounds , which can be prepared by the stepwise or unit construction reactions through the successive addition ML ( L = Cl , Br , Sr , R2 etc ) across six edges or four faces of ME4 ( M = Mo , W ; E = S , Se ) tetrahedra , are described .
	manualset3
167240	8	412731	7	NULL	NULL	NULL	NULL	ME4 ( M = Mo , W ; E = S , Se ) tetrahedra	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The synthetic reactions and spectroscopic studied of molybdenum ( tungsten ) - copper ( silver , iron ) - sulphur ( selenium ) cluster compounds , which can be prepared by the stepwise or unit construction reactions through the successive addition ML ( L = Cl , Br , Sr , R2 etc ) across six edges or four faces of ME4 ( M = Mo , W ; E = S , Se ) tetrahedra , are described .
	manualset3
167241	7	412731	7	NULL	NULL	0	NULL	four faces	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthetic reactions and spectroscopic studied of molybdenum ( tungsten ) - copper ( silver , iron ) - sulphur ( selenium ) cluster compounds , which can be prepared by the stepwise or unit construction reactions through the successive addition ML ( L = Cl , Br , Sr , R2 etc ) across six edges or four faces of ME4 ( M = Mo , W ; E = S , Se ) tetrahedra , are described .
	manualset3
167242	1	412732	7	NULL	NULL	0	NULL	 system 's utility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The system 's utility has been demonstrated by deletion analysis of a chicken myosin heavy chain-encoding gene promoter .
	manualset3
167243	2	412732	7	NULL	NULL	0	NULL	deletion analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The system 's utility has been demonstrated by deletion analysis of a chicken myosin heavy chain-encoding gene promoter .
	manualset3
167244	3	412732	7	NULL	NULL	0	NULL	chicken myosin heavy chain-encoding gene promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The system 's utility has been demonstrated by deletion analysis of a chicken myosin heavy chain-encoding gene promoter .
	manualset3
167245	1	412733	7	NULL	NULL	0	NULL	system operations	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The system operations are controlled by microcontroller ( AT89S52 ) and the main features of the system are software data acquisition , real time LCD display of radiation level , data archiving at removable compact flash card .
	manualset3
167246	2	412733	7	NULL	NULL	0	NULL	microcontroller ( AT89S52 ) 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The system operations are controlled by microcontroller ( AT89S52 ) and the main features of the system are software data acquisition , real time LCD display of radiation level , data archiving at removable compact flash card .
	manualset3
167247	3	412733	7	NULL	NULL	0	NULL	main features	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The system operations are controlled by microcontroller ( AT89S52 ) and the main features of the system are software data acquisition , real time LCD display of radiation level , data archiving at removable compact flash card .
	manualset3
167248	4	412733	7	NULL	NULL	0	NULL	system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The system operations are controlled by microcontroller ( AT89S52 ) and the main features of the system are software data acquisition , real time LCD display of radiation level , data archiving at removable compact flash card .
	manualset3
167249	5	412733	7	NULL	NULL	0	NULL	software data acquisition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The system operations are controlled by microcontroller ( AT89S52 ) and the main features of the system are software data acquisition , real time LCD display of radiation level , data archiving at removable compact flash card .
	manualset3
167250	6	412733	7	NULL	NULL	0	NULL	real time LCD display	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The system operations are controlled by microcontroller ( AT89S52 ) and the main features of the system are software data acquisition , real time LCD display of radiation level , data archiving at removable compact flash card .
	manualset3
167251	7	412733	7	NULL	NULL	0	NULL	radiation level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The system operations are controlled by microcontroller ( AT89S52 ) and the main features of the system are software data acquisition , real time LCD display of radiation level , data archiving at removable compact flash card .
	manualset3
167252	8	412733	7	NULL	NULL	0	NULL	data archiving 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The system operations are controlled by microcontroller ( AT89S52 ) and the main features of the system are software data acquisition , real time LCD display of radiation level , data archiving at removable compact flash card .
	manualset3
167253	9	412733	7	NULL	NULL	0	NULL	compact flash card	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The system operations are controlled by microcontroller ( AT89S52 ) and the main features of the system are software data acquisition , real time LCD display of radiation level , data archiving at removable compact flash card .
	manualset3
167254	1	412734	7	NULL	NULL	0	NULL	system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The system was tested using 296 digitized images of dolphins , representing 94 individual dolphins .
	manualset3
167255	2	412734	7	NULL	NULL	NULL	NULL	296 digitized images	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The system was tested using 296 digitized images of dolphins , representing 94 individual dolphins .
	manualset3
167256	3	412734	7	NULL	NULL	0	NULL	dolphins	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The system was tested using 296 digitized images of dolphins , representing 94 individual dolphins .
	manualset3
167257	4	412734	7	NULL	NULL	NULL	NULL	94 individual dolphins	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The system was tested using 296 digitized images of dolphins , representing 94 individual dolphins .
	manualset3
167259	1	412735	7	NULL	NULL	NULL	NULL	( 3H ) RU 486 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( 3H ) RU 486 competes with dexamethasone for rat kidney glucocorticoid receptor ( GR ) occupancy in vitro , exhibiting a higher association constant for binding to GR than ( 3H ) dexamethasone .
	manualset3
167260	2	412735	7	NULL	NULL	0	NULL	dexamethasone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3H ) RU 486 competes with dexamethasone for rat kidney glucocorticoid receptor ( GR ) occupancy in vitro , exhibiting a higher association constant for binding to GR than ( 3H ) dexamethasone .
	manualset3
167261	3	412735	7	NULL	NULL	0	NULL	 rat kidney glucocorticoid receptor ( GR )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3H ) RU 486 competes with dexamethasone for rat kidney glucocorticoid receptor ( GR ) occupancy in vitro , exhibiting a higher association constant for binding to GR than ( 3H ) dexamethasone .
	manualset3
167262	4	412735	7	NULL	NULL	0	NULL	higher association constant 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3H ) RU 486 competes with dexamethasone for rat kidney glucocorticoid receptor ( GR ) occupancy in vitro , exhibiting a higher association constant for binding to GR than ( 3H ) dexamethasone .
	manualset3
167263	5	412735	7	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3H ) RU 486 competes with dexamethasone for rat kidney glucocorticoid receptor ( GR ) occupancy in vitro , exhibiting a higher association constant for binding to GR than ( 3H ) dexamethasone .
	manualset3
167264	6	412735	7	NULL	NULL	0	NULL	GR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3H ) RU 486 competes with dexamethasone for rat kidney glucocorticoid receptor ( GR ) occupancy in vitro , exhibiting a higher association constant for binding to GR than ( 3H ) dexamethasone .
	manualset3
167265	7	412735	7	NULL	NULL	0	NULL	( 3H ) dexamethasone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3H ) RU 486 competes with dexamethasone for rat kidney glucocorticoid receptor ( GR ) occupancy in vitro , exhibiting a higher association constant for binding to GR than ( 3H ) dexamethasone .
	manualset3
167266	1	412736	7	NULL	NULL	0	NULL	Cohort study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cohort study on mortality among leather and hide tanning workers of the USL 11 area -- Lower Valdarno region ) .
	manualset3
167267	2	412736	7	NULL	NULL	0	NULL	 mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cohort study on mortality among leather and hide tanning workers of the USL 11 area -- Lower Valdarno region ) .
	manualset3
167268	3	412736	7	NULL	NULL	0	NULL	leather and hide tanning workers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cohort study on mortality among leather and hide tanning workers of the USL 11 area -- Lower Valdarno region ) .
	manualset3
167269	4	412736	7	NULL	NULL	0	NULL	 USL 11 area -- Lower Valdarno region	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cohort study on mortality among leather and hide tanning workers of the USL 11 area -- Lower Valdarno region ) .
	manualset3
167270	1	412737	7	NULL	NULL	0	NULL	Acetylcholine-induced relaxation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetylcholine-induced relaxation in both arteries was attenuated , and the attenuation was restored to the control level by indomethacin .
	manualset3
167271	2	412737	7	NULL	NULL	0	NULL	arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetylcholine-induced relaxation in both arteries was attenuated , and the attenuation was restored to the control level by indomethacin .
	manualset3
167272	3	412737	7	NULL	NULL	0	NULL	attenuation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetylcholine-induced relaxation in both arteries was attenuated , and the attenuation was restored to the control level by indomethacin .
	manualset3
167273	4	412737	7	NULL	NULL	0	NULL	control level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetylcholine-induced relaxation in both arteries was attenuated , and the attenuation was restored to the control level by indomethacin .
	manualset3
167274	5	412737	7	NULL	NULL	0	NULL	 indomethacin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetylcholine-induced relaxation in both arteries was attenuated , and the attenuation was restored to the control level by indomethacin .
	manualset3
167275	1	412738	7	NULL	NULL	0	NULL	t ( Lub2 ) chromosome 17 variant	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The t ( Lub2 ) chromosome 17 variant contains a small deletion that removes at least seven genes including Igf2r .
	manualset3
167276	2	412738	7	NULL	NULL	0	NULL	small deletion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The t ( Lub2 ) chromosome 17 variant contains a small deletion that removes at least seven genes including Igf2r .
	manualset3
167277	3	412738	7	NULL	NULL	0	NULL	seven genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The t ( Lub2 ) chromosome 17 variant contains a small deletion that removes at least seven genes including Igf2r .
	manualset3
167278	4	412738	7	NULL	NULL	0	NULL	Igf2r	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The t ( Lub2 ) chromosome 17 variant contains a small deletion that removes at least seven genes including Igf2r .
	manualset3
167279	1	412739	7	NULL	NULL	0	NULL	tachycardia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The tachycardia induced by heptaminol was markedly diminished after pretreatment with reserpine .
	manualset3
167280	2	412739	7	NULL	NULL	NULL	NULL	heptaminol	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The tachycardia induced by heptaminol was markedly diminished after pretreatment with reserpine .
	manualset3
167281	3	412739	7	NULL	NULL	0	NULL	pretreatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The tachycardia induced by heptaminol was markedly diminished after pretreatment with reserpine .
	manualset3
167282	4	412739	7	NULL	NULL	0	NULL	reserpine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The tachycardia induced by heptaminol was markedly diminished after pretreatment with reserpine .
	manualset3
167283	1	412740	7	NULL	NULL	0	NULL	tachykinin NK1 receptor antagonist	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The tachykinin NK1 receptor antagonist , SR 140333 ( 0.1 micromol kg ( -1 ) , i.v. ) , abolished the 2 h PPE response whilst the tachykinin NK2 receptor antagonist MEN 11420 ( 0.1 micromol kg ( -1 ) , i.v. ) appeared to reduce the response by approximately 50 % but this did not reach significance .
	manualset3
167284	2	412740	7	NULL	NULL	0	NULL	SR 140333	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The tachykinin NK1 receptor antagonist , SR 140333 ( 0.1 micromol kg ( -1 ) , i.v. ) , abolished the 2 h PPE response whilst the tachykinin NK2 receptor antagonist MEN 11420 ( 0.1 micromol kg ( -1 ) , i.v. ) appeared to reduce the response by approximately 50 % but this did not reach significance .
	manualset3
167285	3	412740	7	NULL	NULL	0	NULL	0.1 micromol kg ( -1 ) , i.v.	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The tachykinin NK1 receptor antagonist , SR 140333 ( 0.1 micromol kg ( -1 ) , i.v. ) , abolished the 2 h PPE response whilst the tachykinin NK2 receptor antagonist MEN 11420 ( 0.1 micromol kg ( -1 ) , i.v. ) appeared to reduce the response by approximately 50 % but this did not reach significance .
	manualset3
167286	4	412740	7	NULL	NULL	NULL	NULL	 PPE response	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The tachykinin NK1 receptor antagonist , SR 140333 ( 0.1 micromol kg ( -1 ) , i.v. ) , abolished the 2 h PPE response whilst the tachykinin NK2 receptor antagonist MEN 11420 ( 0.1 micromol kg ( -1 ) , i.v. ) appeared to reduce the response by approximately 50 % but this did not reach significance .
	manualset3
167287	5	412740	7	NULL	NULL	0	NULL	tachykinin NK2 receptor antagonist MEN 11420	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The tachykinin NK1 receptor antagonist , SR 140333 ( 0.1 micromol kg ( -1 ) , i.v. ) , abolished the 2 h PPE response whilst the tachykinin NK2 receptor antagonist MEN 11420 ( 0.1 micromol kg ( -1 ) , i.v. ) appeared to reduce the response by approximately 50 % but this did not reach significance .
	manualset3
167288	6	412740	7	NULL	NULL	0	NULL	0.1 micromol kg ( -1 ) , i.v.	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The tachykinin NK1 receptor antagonist , SR 140333 ( 0.1 micromol kg ( -1 ) , i.v. ) , abolished the 2 h PPE response whilst the tachykinin NK2 receptor antagonist MEN 11420 ( 0.1 micromol kg ( -1 ) , i.v. ) appeared to reduce the response by approximately 50 % but this did not reach significance .
	manualset3
167289	7	412740	7	NULL	NULL	NULL	NULL	response	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The tachykinin NK1 receptor antagonist , SR 140333 ( 0.1 micromol kg ( -1 ) , i.v. ) , abolished the 2 h PPE response whilst the tachykinin NK2 receptor antagonist MEN 11420 ( 0.1 micromol kg ( -1 ) , i.v. ) appeared to reduce the response by approximately 50 % but this did not reach significance .
	manualset3
167290	8	412740	7	NULL	NULL	0	NULL	50 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The tachykinin NK1 receptor antagonist , SR 140333 ( 0.1 micromol kg ( -1 ) , i.v. ) , abolished the 2 h PPE response whilst the tachykinin NK2 receptor antagonist MEN 11420 ( 0.1 micromol kg ( -1 ) , i.v. ) appeared to reduce the response by approximately 50 % but this did not reach significance .
	manualset3
168348	9	412740	7	NULL	NULL	0	NULL	2 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The tachykinin NK1 receptor antagonist , SR 140333 ( 0.1 micromol kg ( -1 ) , i.v. ) , abolished the 2 h PPE response whilst the tachykinin NK2 receptor antagonist MEN 11420 ( 0.1 micromol kg ( -1 ) , i.v. ) appeared to reduce the response by approximately 50 % but this did not reach significance .
	manualset3
169181	10	412740	7	NULL	NULL	0	NULL	significance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The tachykinin NK1 receptor antagonist , SR 140333 ( 0.1 micromol kg ( -1 ) , i.v. ) , abolished the 2 h PPE response whilst the tachykinin NK2 receptor antagonist MEN 11420 ( 0.1 micromol kg ( -1 ) , i.v. ) appeared to reduce the response by approximately 50 % but this did not reach significance .
	manualset3
167291	1	412741	7	NULL	NULL	0	NULL	target Hb concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The target Hb concentration 11-12 g/dL is maintained in 90-95 % of the patients by administering 1.000-30 .000 IU of epoetin ( 5-150 mcg darbepoetin alpha ) per week in the presence of adequate reserves of iron .
	manualset3
167292	2	412741	7	NULL	NULL	0	NULL	11-12 g/dL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The target Hb concentration 11-12 g/dL is maintained in 90-95 % of the patients by administering 1.000-30 .000 IU of epoetin ( 5-150 mcg darbepoetin alpha ) per week in the presence of adequate reserves of iron .
	manualset3
167293	3	412741	7	NULL	NULL	0	NULL	90-95 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The target Hb concentration 11-12 g/dL is maintained in 90-95 % of the patients by administering 1.000-30 .000 IU of epoetin ( 5-150 mcg darbepoetin alpha ) per week in the presence of adequate reserves of iron .
	manualset3
167294	4	412741	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The target Hb concentration 11-12 g/dL is maintained in 90-95 % of the patients by administering 1.000-30 .000 IU of epoetin ( 5-150 mcg darbepoetin alpha ) per week in the presence of adequate reserves of iron .
	manualset3
167295	5	412741	7	NULL	NULL	NULL	NULL	1.000-30 .000 IU	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The target Hb concentration 11-12 g/dL is maintained in 90-95 % of the patients by administering 1.000-30 .000 IU of epoetin ( 5-150 mcg darbepoetin alpha ) per week in the presence of adequate reserves of iron .
	manualset3
167296	6	412741	7	NULL	NULL	0	NULL	epoetin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The target Hb concentration 11-12 g/dL is maintained in 90-95 % of the patients by administering 1.000-30 .000 IU of epoetin ( 5-150 mcg darbepoetin alpha ) per week in the presence of adequate reserves of iron .
	manualset3
167297	7	412741	7	NULL	NULL	NULL	NULL	5-150 mcg per week	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The target Hb concentration 11-12 g/dL is maintained in 90-95 % of the patients by administering 1.000-30 .000 IU of epoetin ( 5-150 mcg darbepoetin alpha ) per week in the presence of adequate reserves of iron .
	manualset3
167298	8	412741	7	NULL	NULL	0	NULL	darbepoetin alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The target Hb concentration 11-12 g/dL is maintained in 90-95 % of the patients by administering 1.000-30 .000 IU of epoetin ( 5-150 mcg darbepoetin alpha ) per week in the presence of adequate reserves of iron .
	manualset3
167299	9	412741	7	NULL	NULL	0	NULL	presence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The target Hb concentration 11-12 g/dL is maintained in 90-95 % of the patients by administering 1.000-30 .000 IU of epoetin ( 5-150 mcg darbepoetin alpha ) per week in the presence of adequate reserves of iron .
	manualset3
167300	10	412741	7	NULL	NULL	NULL	NULL	adequate reserves	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The target Hb concentration 11-12 g/dL is maintained in 90-95 % of the patients by administering 1.000-30 .000 IU of epoetin ( 5-150 mcg darbepoetin alpha ) per week in the presence of adequate reserves of iron .
	manualset3
167301	11	412741	7	NULL	NULL	0	NULL	iron	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The target Hb concentration 11-12 g/dL is maintained in 90-95 % of the patients by administering 1.000-30 .000 IU of epoetin ( 5-150 mcg darbepoetin alpha ) per week in the presence of adequate reserves of iron .
	manualset3
167302	1	412742	7	NULL	NULL	0	NULL	 target cell specificity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The target cell specificity of LKT for bovine leukocytic cells was retained by the SDS-PAGE LKT , and isolated LPS at comparable concentrations to that in CCS LKT exhibited no leukolytic activity .
	manualset3
167303	2	412742	7	NULL	NULL	0	NULL	LKT	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The target cell specificity of LKT for bovine leukocytic cells was retained by the SDS-PAGE LKT , and isolated LPS at comparable concentrations to that in CCS LKT exhibited no leukolytic activity .
	manualset3
167304	3	412742	7	NULL	NULL	0	NULL	bovine leukocytic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The target cell specificity of LKT for bovine leukocytic cells was retained by the SDS-PAGE LKT , and isolated LPS at comparable concentrations to that in CCS LKT exhibited no leukolytic activity .
	manualset3
167305	4	412742	7	NULL	NULL	0	NULL	 SDS-PAGE LKT	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The target cell specificity of LKT for bovine leukocytic cells was retained by the SDS-PAGE LKT , and isolated LPS at comparable concentrations to that in CCS LKT exhibited no leukolytic activity .
	manualset3
167306	5	412742	7	NULL	NULL	0	NULL	 isolated LPS	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The target cell specificity of LKT for bovine leukocytic cells was retained by the SDS-PAGE LKT , and isolated LPS at comparable concentrations to that in CCS LKT exhibited no leukolytic activity .
	manualset3
167307	6	412742	7	NULL	NULL	0	NULL	concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The target cell specificity of LKT for bovine leukocytic cells was retained by the SDS-PAGE LKT , and isolated LPS at comparable concentrations to that in CCS LKT exhibited no leukolytic activity .
	manualset3
167308	7	412742	7	NULL	NULL	0	NULL	CCS LKT	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The target cell specificity of LKT for bovine leukocytic cells was retained by the SDS-PAGE LKT , and isolated LPS at comparable concentrations to that in CCS LKT exhibited no leukolytic activity .
	manualset3
167309	8	412742	7	NULL	NULL	0	NULL	leukolytic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The target cell specificity of LKT for bovine leukocytic cells was retained by the SDS-PAGE LKT , and isolated LPS at comparable concentrations to that in CCS LKT exhibited no leukolytic activity .
	manualset3
167310	1	412743	7	NULL	NULL	0	NULL	target compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The target compounds were analyzed in solvent and in two representative food matrices such as cucumber ( high water content ) and egg ( high fat content ) .
	manualset3
167311	2	412743	7	NULL	NULL	0	NULL	solvent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The target compounds were analyzed in solvent and in two representative food matrices such as cucumber ( high water content ) and egg ( high fat content ) .
	manualset3
167312	3	412743	7	NULL	NULL	0	NULL	two	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The target compounds were analyzed in solvent and in two representative food matrices such as cucumber ( high water content ) and egg ( high fat content ) .
	manualset3
167313	4	412743	7	NULL	NULL	0	NULL	food matrices 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The target compounds were analyzed in solvent and in two representative food matrices such as cucumber ( high water content ) and egg ( high fat content ) .
	manualset3
167314	5	412743	7	NULL	NULL	0	NULL	cucumber	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The target compounds were analyzed in solvent and in two representative food matrices such as cucumber ( high water content ) and egg ( high fat content ) .
	manualset3
167315	6	412743	7	NULL	NULL	0	NULL	high water content	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The target compounds were analyzed in solvent and in two representative food matrices such as cucumber ( high water content ) and egg ( high fat content ) .
	manualset3
167316	7	412743	7	NULL	NULL	0	NULL	egg	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The target compounds were analyzed in solvent and in two representative food matrices such as cucumber ( high water content ) and egg ( high fat content ) .
	manualset3
167317	8	412743	7	NULL	NULL	0	NULL	high fat content 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The target compounds were analyzed in solvent and in two representative food matrices such as cucumber ( high water content ) and egg ( high fat content ) .
	manualset3
167318	1	412744	7	NULL	NULL	0	NULL	 target	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The target of this study was to describe the interactions between body condition and various descriptors of yield and fertility .
	manualset3
167319	2	412744	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The target of this study was to describe the interactions between body condition and various descriptors of yield and fertility .
	manualset3
167320	3	412744	7	NULL	NULL	0	NULL	 interactions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The target of this study was to describe the interactions between body condition and various descriptors of yield and fertility .
	manualset3
167321	4	412744	7	NULL	NULL	0	NULL	body condition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The target of this study was to describe the interactions between body condition and various descriptors of yield and fertility .
	manualset3
167322	5	412744	7	NULL	NULL	0	NULL	descriptors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The target of this study was to describe the interactions between body condition and various descriptors of yield and fertility .
	manualset3
167323	6	412744	7	NULL	NULL	0	NULL	yield	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The target of this study was to describe the interactions between body condition and various descriptors of yield and fertility .
	manualset3
167324	7	412744	7	NULL	NULL	0	NULL	fertility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The target of this study was to describe the interactions between body condition and various descriptors of yield and fertility .
	manualset3
167325	1	412745	7	NULL	NULL	0	NULL	team 's other novel findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The team 's other novel findings included a delay in the normal fall in pulmonary vascular resistance after birth and , in adults , a lack of vasodilation with muscular exercise .
	manualset3
167326	2	412745	7	NULL	NULL	0	NULL	delay	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The team 's other novel findings included a delay in the normal fall in pulmonary vascular resistance after birth and , in adults , a lack of vasodilation with muscular exercise .
	manualset3
167327	3	412745	7	NULL	NULL	0	NULL	normal fall	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The team 's other novel findings included a delay in the normal fall in pulmonary vascular resistance after birth and , in adults , a lack of vasodilation with muscular exercise .
	manualset3
167328	4	412745	7	NULL	NULL	0	NULL	 pulmonary vascular resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The team 's other novel findings included a delay in the normal fall in pulmonary vascular resistance after birth and , in adults , a lack of vasodilation with muscular exercise .
	manualset3
167329	5	412745	7	NULL	NULL	0	NULL	 birth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The team 's other novel findings included a delay in the normal fall in pulmonary vascular resistance after birth and , in adults , a lack of vasodilation with muscular exercise .
	manualset3
167330	6	412745	7	NULL	NULL	0	NULL	adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The team 's other novel findings included a delay in the normal fall in pulmonary vascular resistance after birth and , in adults , a lack of vasodilation with muscular exercise .
	manualset3
167331	7	412745	7	NULL	NULL	0	NULL	 lack of vasodilation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The team 's other novel findings included a delay in the normal fall in pulmonary vascular resistance after birth and , in adults , a lack of vasodilation with muscular exercise .
	manualset3
167332	8	412745	7	NULL	NULL	0	NULL	muscular exercise	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The team 's other novel findings included a delay in the normal fall in pulmonary vascular resistance after birth and , in adults , a lack of vasodilation with muscular exercise .
	manualset3
167333	1	412746	7	NULL	NULL	0	NULL	 technician	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The technician was able to select previously scored crypts 95 % of the time .
	manualset3
167334	2	412746	7	NULL	NULL	0	NULL	crypts	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The technician was able to select previously scored crypts 95 % of the time .
	manualset3
167335	3	412746	7	NULL	NULL	0	NULL	95 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The technician was able to select previously scored crypts 95 % of the time .
	manualset3
167336	4	412746	7	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The technician was able to select previously scored crypts 95 % of the time .
	manualset3
167337	1	412747	7	NULL	NULL	0	NULL	technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique , using a methylcellulose-based test meal , is simple , versatile and reliable .
	manualset3
167338	2	412747	7	NULL	NULL	0	NULL	methylcellulose-based test meal	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique , using a methylcellulose-based test meal , is simple , versatile and reliable .
	manualset3
167339	1	412748	7	NULL	NULL	0	NULL	 technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique described in this paper requires no digitisation of anatomical features or fiducial markers but instead relies on image matching between pseudo and real x-ray images generated by a virtual and a real image intensifier respectively .
	manualset3
167340	2	412748	7	NULL	NULL	0	NULL	 paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique described in this paper requires no digitisation of anatomical features or fiducial markers but instead relies on image matching between pseudo and real x-ray images generated by a virtual and a real image intensifier respectively .
	manualset3
167341	3	412748	7	NULL	NULL	0	NULL	digitisation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique described in this paper requires no digitisation of anatomical features or fiducial markers but instead relies on image matching between pseudo and real x-ray images generated by a virtual and a real image intensifier respectively .
	manualset3
167342	4	412748	7	NULL	NULL	0	NULL	anatomical features	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique described in this paper requires no digitisation of anatomical features or fiducial markers but instead relies on image matching between pseudo and real x-ray images generated by a virtual and a real image intensifier respectively .
	manualset3
167343	5	412748	7	NULL	NULL	0	NULL	fiducial markers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique described in this paper requires no digitisation of anatomical features or fiducial markers but instead relies on image matching between pseudo and real x-ray images generated by a virtual and a real image intensifier respectively .
	manualset3
167344	6	412748	7	NULL	NULL	0	NULL	image matching	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique described in this paper requires no digitisation of anatomical features or fiducial markers but instead relies on image matching between pseudo and real x-ray images generated by a virtual and a real image intensifier respectively .
	manualset3
167345	7	412748	7	NULL	NULL	NULL	NULL	pseudo x-ray images	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The technique described in this paper requires no digitisation of anatomical features or fiducial markers but instead relies on image matching between pseudo and real x-ray images generated by a virtual and a real image intensifier respectively .
	manualset3
167346	8	412748	7	NULL	NULL	NULL	NULL	real x-ray images	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The technique described in this paper requires no digitisation of anatomical features or fiducial markers but instead relies on image matching between pseudo and real x-ray images generated by a virtual and a real image intensifier respectively .
	manualset3
167347	9	412748	7	NULL	NULL	NULL	NULL	 virtual image intensifier	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The technique described in this paper requires no digitisation of anatomical features or fiducial markers but instead relies on image matching between pseudo and real x-ray images generated by a virtual and a real image intensifier respectively .
	manualset3
167348	10	412748	7	NULL	NULL	NULL	NULL	 real image intensifier	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The technique described in this paper requires no digitisation of anatomical features or fiducial markers but instead relies on image matching between pseudo and real x-ray images generated by a virtual and a real image intensifier respectively .
	manualset3
167349	1	412749	7	NULL	NULL	0	NULL	technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique is based on enamel microabrasion with application of an acid-abrasive gel .
	manualset3
167350	2	412749	7	NULL	NULL	0	NULL	enamel microabrasion	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique is based on enamel microabrasion with application of an acid-abrasive gel .
	manualset3
167351	3	412749	7	NULL	NULL	0	NULL	 application 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique is based on enamel microabrasion with application of an acid-abrasive gel .
	manualset3
167352	4	412749	7	NULL	NULL	0	NULL	acid-abrasive gel	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique is based on enamel microabrasion with application of an acid-abrasive gel .
	manualset3
167353	1	412750	7	NULL	NULL	0	NULL	technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique is deemed quite reliable and robust , as this is illustrated by a very good agreement between the extracted contor and the expert manual drawing output .
	manualset3
167354	2	412750	7	NULL	NULL	0	NULL	 agreement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique is deemed quite reliable and robust , as this is illustrated by a very good agreement between the extracted contor and the expert manual drawing output .
	manualset3
167355	3	412750	7	NULL	NULL	0	NULL	extracted contor	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique is deemed quite reliable and robust , as this is illustrated by a very good agreement between the extracted contor and the expert manual drawing output .
	manualset3
167356	4	412750	7	NULL	NULL	0	NULL	expert manual drawing output	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique is deemed quite reliable and robust , as this is illustrated by a very good agreement between the extracted contor and the expert manual drawing output .
	manualset3
167357	1	412751	7	NULL	NULL	0	NULL	technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique is described in detail and includes tightly packing cancellous bone chips about an intramedullary stem and into the periprosthetic bone defects , then fully cementing a component in place .
	manualset3
167358	2	412751	7	NULL	NULL	0	NULL	tightly packing cancellous bone chips	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique is described in detail and includes tightly packing cancellous bone chips about an intramedullary stem and into the periprosthetic bone defects , then fully cementing a component in place .
	manualset3
167359	3	412751	7	NULL	NULL	0	NULL	intramedullary stem	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique is described in detail and includes tightly packing cancellous bone chips about an intramedullary stem and into the periprosthetic bone defects , then fully cementing a component in place .
	manualset3
167360	4	412751	7	NULL	NULL	0	NULL	periprosthetic bone defects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique is described in detail and includes tightly packing cancellous bone chips about an intramedullary stem and into the periprosthetic bone defects , then fully cementing a component in place .
	manualset3
167361	5	412751	7	NULL	NULL	0	NULL	component	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique is described in detail and includes tightly packing cancellous bone chips about an intramedullary stem and into the periprosthetic bone defects , then fully cementing a component in place .
	manualset3
167362	1	412752	7	NULL	NULL	0	NULL	 technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique is extended to three dimensions such that the entire symmetric elasticity tensor is assessed .
	manualset3
167363	2	412752	7	NULL	NULL	0	NULL	three dimensions	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique is extended to three dimensions such that the entire symmetric elasticity tensor is assessed .
	manualset3
167364	3	412752	7	NULL	NULL	0	NULL	symmetric elasticity tensor	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique is extended to three dimensions such that the entire symmetric elasticity tensor is assessed .
	manualset3
167365	1	412753	7	NULL	NULL	0	NULL	 technique 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique of parameter estimation was used to calculate optimal values for responses from human subjects in which saccadic and convergence components of response were either nearly synchronized or temporally dissociated .
	manualset3
167366	2	412753	7	NULL	NULL	0	NULL	parameter estimation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique of parameter estimation was used to calculate optimal values for responses from human subjects in which saccadic and convergence components of response were either nearly synchronized or temporally dissociated .
	manualset3
167367	3	412753	7	NULL	NULL	0	NULL	optimal values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique of parameter estimation was used to calculate optimal values for responses from human subjects in which saccadic and convergence components of response were either nearly synchronized or temporally dissociated .
	manualset3
167368	4	412753	7	NULL	NULL	0	NULL	 responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique of parameter estimation was used to calculate optimal values for responses from human subjects in which saccadic and convergence components of response were either nearly synchronized or temporally dissociated .
	manualset3
167369	5	412753	7	NULL	NULL	0	NULL	human subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique of parameter estimation was used to calculate optimal values for responses from human subjects in which saccadic and convergence components of response were either nearly synchronized or temporally dissociated .
	manualset3
167370	6	412753	7	NULL	NULL	0	NULL	 saccadic components	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique of parameter estimation was used to calculate optimal values for responses from human subjects in which saccadic and convergence components of response were either nearly synchronized or temporally dissociated .
	manualset3
167371	7	412753	7	NULL	NULL	0	NULL	convergence components	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique of parameter estimation was used to calculate optimal values for responses from human subjects in which saccadic and convergence components of response were either nearly synchronized or temporally dissociated .
	manualset3
167372	8	412753	7	NULL	NULL	0	NULL	response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique of parameter estimation was used to calculate optimal values for responses from human subjects in which saccadic and convergence components of response were either nearly synchronized or temporally dissociated .
	manualset3
167373	1	412754	7	NULL	NULL	NULL	NULL	technique 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The technique of translumbar inferior vena cava central venous access is described in a critically ill child .
	manualset3
167374	2	412754	7	NULL	NULL	0	NULL	translumbar inferior vena cava central venous access	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique of translumbar inferior vena cava central venous access is described in a critically ill child .
	manualset3
167375	3	412754	7	NULL	NULL	0	NULL	 ill child	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique of translumbar inferior vena cava central venous access is described in a critically ill child .
	manualset3
167376	1	412755	7	NULL	NULL	NULL	NULL	 technique	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The technique proved to be sound , offering safe conditions for both mother and foetus , and absence of noteworthy side-effects , and a good post-operative analgesic effect .
	manualset3
167377	2	412755	7	NULL	NULL	0	NULL	safe conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique proved to be sound , offering safe conditions for both mother and foetus , and absence of noteworthy side-effects , and a good post-operative analgesic effect .
	manualset3
167378	3	412755	7	NULL	NULL	0	NULL	mother	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique proved to be sound , offering safe conditions for both mother and foetus , and absence of noteworthy side-effects , and a good post-operative analgesic effect .
	manualset3
167379	4	412755	7	NULL	NULL	0	NULL	 foetus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique proved to be sound , offering safe conditions for both mother and foetus , and absence of noteworthy side-effects , and a good post-operative analgesic effect .
	manualset3
167380	5	412755	7	NULL	NULL	0	NULL	absence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique proved to be sound , offering safe conditions for both mother and foetus , and absence of noteworthy side-effects , and a good post-operative analgesic effect .
	manualset3
167381	6	412755	7	NULL	NULL	0	NULL	side-effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique proved to be sound , offering safe conditions for both mother and foetus , and absence of noteworthy side-effects , and a good post-operative analgesic effect .
	manualset3
167382	7	412755	7	NULL	NULL	0	NULL	post-operative analgesic effect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique proved to be sound , offering safe conditions for both mother and foetus , and absence of noteworthy side-effects , and a good post-operative analgesic effect .
	manualset3
167383	1	412756	7	NULL	NULL	0	NULL	 technique 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique uses rigid steel wires passed through both abdominal thicknesses perpendicularly to the incision with an extraperitoneal course and passed through a large Silastic tube laid on the skin surface parallel to the incision .
	manualset3
167384	2	412756	7	NULL	NULL	0	NULL	 rigid steel wires	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique uses rigid steel wires passed through both abdominal thicknesses perpendicularly to the incision with an extraperitoneal course and passed through a large Silastic tube laid on the skin surface parallel to the incision .
	manualset3
167385	3	412756	7	NULL	NULL	0	NULL	abdominal thicknesses	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique uses rigid steel wires passed through both abdominal thicknesses perpendicularly to the incision with an extraperitoneal course and passed through a large Silastic tube laid on the skin surface parallel to the incision .
	manualset3
167386	4	412756	7	NULL	NULL	0	NULL	incision	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique uses rigid steel wires passed through both abdominal thicknesses perpendicularly to the incision with an extraperitoneal course and passed through a large Silastic tube laid on the skin surface parallel to the incision .
	manualset3
167387	5	412756	7	NULL	NULL	0	NULL	extraperitoneal course	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique uses rigid steel wires passed through both abdominal thicknesses perpendicularly to the incision with an extraperitoneal course and passed through a large Silastic tube laid on the skin surface parallel to the incision .
	manualset3
167388	6	412756	7	NULL	NULL	0	NULL	large Silastic tube	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique uses rigid steel wires passed through both abdominal thicknesses perpendicularly to the incision with an extraperitoneal course and passed through a large Silastic tube laid on the skin surface parallel to the incision .
	manualset3
167389	7	412756	7	NULL	NULL	0	NULL	skin surface	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique uses rigid steel wires passed through both abdominal thicknesses perpendicularly to the incision with an extraperitoneal course and passed through a large Silastic tube laid on the skin surface parallel to the incision .
	manualset3
167390	8	412756	7	NULL	NULL	0	NULL	 incision 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique uses rigid steel wires passed through both abdominal thicknesses perpendicularly to the incision with an extraperitoneal course and passed through a large Silastic tube laid on the skin surface parallel to the incision .
	manualset3
167391	1	412757	7	NULL	NULL	0	NULL	Acetylcholinesterase activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetylcholinesterase activity of approximately 80 % of both populations was not inhibited by a standard dosage of propoxur .
	manualset3
167392	2	412757	7	NULL	NULL	0	NULL	80 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetylcholinesterase activity of approximately 80 % of both populations was not inhibited by a standard dosage of propoxur .
	manualset3
167393	3	412757	7	NULL	NULL	0	NULL	populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetylcholinesterase activity of approximately 80 % of both populations was not inhibited by a standard dosage of propoxur .
	manualset3
167394	4	412757	7	NULL	NULL	0	NULL	standard dosage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetylcholinesterase activity of approximately 80 % of both populations was not inhibited by a standard dosage of propoxur .
	manualset3
167395	5	412757	7	NULL	NULL	0	NULL	propoxur	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetylcholinesterase activity of approximately 80 % of both populations was not inhibited by a standard dosage of propoxur .
	manualset3
167396	1	412758	7	NULL	NULL	0	NULL	techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The techniques enabled us to detect lectin binding sites in the various intracellular compartments of photoreceptor cells , retinal pigment epithelium ( RPE ) , and interphotoreceptor matrices .
	manualset3
167397	2	412758	7	NULL	NULL	0	NULL	lectin binding sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The techniques enabled us to detect lectin binding sites in the various intracellular compartments of photoreceptor cells , retinal pigment epithelium ( RPE ) , and interphotoreceptor matrices .
	manualset3
167398	3	412758	7	NULL	NULL	0	NULL	intracellular compartments	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The techniques enabled us to detect lectin binding sites in the various intracellular compartments of photoreceptor cells , retinal pigment epithelium ( RPE ) , and interphotoreceptor matrices .
	manualset3
167399	4	412758	7	NULL	NULL	0	NULL	photoreceptor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The techniques enabled us to detect lectin binding sites in the various intracellular compartments of photoreceptor cells , retinal pigment epithelium ( RPE ) , and interphotoreceptor matrices .
	manualset3
167400	5	412758	7	NULL	NULL	NULL	NULL	retinal pigment epithelium ( RPE )	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The techniques enabled us to detect lectin binding sites in the various intracellular compartments of photoreceptor cells , retinal pigment epithelium ( RPE ) , and interphotoreceptor matrices .
	manualset3
167401	6	412758	7	NULL	NULL	NULL	NULL	interphotoreceptor matrices	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The techniques enabled us to detect lectin binding sites in the various intracellular compartments of photoreceptor cells , retinal pigment epithelium ( RPE ) , and interphotoreceptor matrices .
	manualset3
167402	1	412759	7	NULL	NULL	0	NULL	techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The techniques were applied to fura-2-labeled astroglial cells in primary culture exposed to hypo - or hyperosmotic stress .
	manualset3
167403	2	412759	7	NULL	NULL	0	NULL	fura-2-labeled astroglial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The techniques were applied to fura-2-labeled astroglial cells in primary culture exposed to hypo - or hyperosmotic stress .
	manualset3
167404	3	412759	7	NULL	NULL	0	NULL	primary culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The techniques were applied to fura-2-labeled astroglial cells in primary culture exposed to hypo - or hyperosmotic stress .
	manualset3
167405	4	412759	7	NULL	NULL	NULL	NULL	hypoosmotic stress	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The techniques were applied to fura-2-labeled astroglial cells in primary culture exposed to hypo - or hyperosmotic stress .
	manualset3
167406	5	412759	7	NULL	NULL	NULL	NULL	hyperosmotic stress	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The techniques were applied to fura-2-labeled astroglial cells in primary culture exposed to hypo - or hyperosmotic stress .
	manualset3
167407	1	412760	7	NULL	NULL	0	NULL	technology	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The technology of fertility control has made dramatic strides in the past 25 years , offering a wider variety of safe , effective contraceptive choices than ever before .
	manualset3
167408	2	412760	7	NULL	NULL	0	NULL	fertility control	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The technology of fertility control has made dramatic strides in the past 25 years , offering a wider variety of safe , effective contraceptive choices than ever before .
	manualset3
167409	3	412760	7	NULL	NULL	NULL	NULL	25 years	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The technology of fertility control has made dramatic strides in the past 25 years , offering a wider variety of safe , effective contraceptive choices than ever before .
	manualset3
167410	4	412760	7	NULL	NULL	NULL	NULL	contraceptive choices	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The technology of fertility control has made dramatic strides in the past 25 years , offering a wider variety of safe , effective contraceptive choices than ever before .
	manualset3
173651	5	412760	7	NULL	NULL	0	NULL	dramatic strides	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The technology of fertility control has made dramatic strides in the past 25 years , offering a wider variety of safe , effective contraceptive choices than ever before .
	manualset3
167411	1	412761	7	NULL	NULL	NULL	NULL	temperature	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The temperature does not great influence on the adsorption isotherm .
	manualset3
167412	2	412761	7	NULL	NULL	0	NULL	adsorption isotherm 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The temperature does not great influence on the adsorption isotherm .
	manualset3
167413	1	412762	7	NULL	NULL	NULL	NULL	 temperature	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The temperature had a strong influence on the biosorption process .
	manualset3
167414	2	412762	7	NULL	NULL	0	NULL	biosorption process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The temperature had a strong influence on the biosorption process .
	manualset3
167415	1	412763	7	NULL	NULL	0	NULL	temporal bone	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The temporal bone often falls within the field of radiation for head and neck tumors .
	manualset3
167416	2	412763	7	NULL	NULL	NULL	NULL	field	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The temporal bone often falls within the field of radiation for head and neck tumors .
	manualset3
167417	3	412763	7	NULL	NULL	0	NULL	radiation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The temporal bone often falls within the field of radiation for head and neck tumors .
	manualset3
167418	4	412763	7	NULL	NULL	NULL	NULL	head and neck tumors	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The temporal bone often falls within the field of radiation for head and neck tumors .
	manualset3
167419	1	412764	7	NULL	NULL	0	NULL	temporal modulation	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The temporal modulation of the heterodyne signal gives the spectrum of the input signal with linear characteristics .
	manualset3
167420	2	412764	7	NULL	NULL	0	NULL	heterodyne signal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The temporal modulation of the heterodyne signal gives the spectrum of the input signal with linear characteristics .
	manualset3
167421	3	412764	7	NULL	NULL	0	NULL	 spectrum 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The temporal modulation of the heterodyne signal gives the spectrum of the input signal with linear characteristics .
	manualset3
167422	4	412764	7	NULL	NULL	0	NULL	 input signal	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The temporal modulation of the heterodyne signal gives the spectrum of the input signal with linear characteristics .
	manualset3
167423	5	412764	7	NULL	NULL	0	NULL	linear characteristics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The temporal modulation of the heterodyne signal gives the spectrum of the input signal with linear characteristics .
	manualset3
167424	1	412765	7	NULL	NULL	0	NULL	temporary increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The temporary increase of calcium level and decrease of inorganic phosphorus in these animals was accompanied by a lower activity of alkaline phosphatase .
	manualset3
167425	2	412765	7	NULL	NULL	0	NULL	calcium level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The temporary increase of calcium level and decrease of inorganic phosphorus in these animals was accompanied by a lower activity of alkaline phosphatase .
	manualset3
167426	3	412765	7	NULL	NULL	0	NULL	 decrease	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The temporary increase of calcium level and decrease of inorganic phosphorus in these animals was accompanied by a lower activity of alkaline phosphatase .
	manualset3
167427	4	412765	7	NULL	NULL	0	NULL	inorganic phosphorus	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The temporary increase of calcium level and decrease of inorganic phosphorus in these animals was accompanied by a lower activity of alkaline phosphatase .
	manualset3
167428	5	412765	7	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The temporary increase of calcium level and decrease of inorganic phosphorus in these animals was accompanied by a lower activity of alkaline phosphatase .
	manualset3
167429	6	412765	7	NULL	NULL	0	NULL	 lower activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The temporary increase of calcium level and decrease of inorganic phosphorus in these animals was accompanied by a lower activity of alkaline phosphatase .
	manualset3
167430	7	412765	7	NULL	NULL	0	NULL	alkaline phosphatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The temporary increase of calcium level and decrease of inorganic phosphorus in these animals was accompanied by a lower activity of alkaline phosphatase .
	manualset3
167431	1	412766	7	NULL	NULL	0	NULL	tensile bond strength	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The tensile bond strength of the resin to the glass plate treated with bisfunctional silane alone was high ( about 20MPa ) in spite of the fact that the molecule contains no double bonds .
	manualset3
167432	2	412766	7	NULL	NULL	0	NULL	resin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The tensile bond strength of the resin to the glass plate treated with bisfunctional silane alone was high ( about 20MPa ) in spite of the fact that the molecule contains no double bonds .
	manualset3
167433	3	412766	7	NULL	NULL	0	NULL	glass plate	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The tensile bond strength of the resin to the glass plate treated with bisfunctional silane alone was high ( about 20MPa ) in spite of the fact that the molecule contains no double bonds .
	manualset3
167434	4	412766	7	NULL	NULL	0	NULL	bisfunctional silane	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The tensile bond strength of the resin to the glass plate treated with bisfunctional silane alone was high ( about 20MPa ) in spite of the fact that the molecule contains no double bonds .
	manualset3
167435	5	412766	7	NULL	NULL	0	NULL	20MPa	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The tensile bond strength of the resin to the glass plate treated with bisfunctional silane alone was high ( about 20MPa ) in spite of the fact that the molecule contains no double bonds .
	manualset3
167436	6	412766	7	NULL	NULL	0	NULL	molecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The tensile bond strength of the resin to the glass plate treated with bisfunctional silane alone was high ( about 20MPa ) in spite of the fact that the molecule contains no double bonds .
	manualset3
167437	7	412766	7	NULL	NULL	0	NULL	 double bonds	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The tensile bond strength of the resin to the glass plate treated with bisfunctional silane alone was high ( about 20MPa ) in spite of the fact that the molecule contains no double bonds .
	manualset3
167438	1	412767	7	NULL	NULL	0	NULL	Aceylcholine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Aceylcholine , 5-HY and prostaglandins appear to play little or no important role in the peripheral airway constrictions to honey bee venom in cat .
	manualset3
167439	2	412767	7	NULL	NULL	0	NULL	5-HY 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Aceylcholine , 5-HY and prostaglandins appear to play little or no important role in the peripheral airway constrictions to honey bee venom in cat .
	manualset3
167440	3	412767	7	NULL	NULL	0	NULL	prostaglandins	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Aceylcholine , 5-HY and prostaglandins appear to play little or no important role in the peripheral airway constrictions to honey bee venom in cat .
	manualset3
167441	4	412767	7	NULL	NULL	0	NULL	 role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Aceylcholine , 5-HY and prostaglandins appear to play little or no important role in the peripheral airway constrictions to honey bee venom in cat .
	manualset3
167442	5	412767	7	NULL	NULL	0	NULL	 peripheral airway constrictions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Aceylcholine , 5-HY and prostaglandins appear to play little or no important role in the peripheral airway constrictions to honey bee venom in cat .
	manualset3
167443	6	412767	7	NULL	NULL	0	NULL	 honey bee venom	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Aceylcholine , 5-HY and prostaglandins appear to play little or no important role in the peripheral airway constrictions to honey bee venom in cat .
	manualset3
167444	7	412767	7	NULL	NULL	0	NULL	cat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Aceylcholine , 5-HY and prostaglandins appear to play little or no important role in the peripheral airway constrictions to honey bee venom in cat .
	manualset3
167445	1	412768	7	NULL	NULL	0	NULL	 tension 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The tension must be maintained for the good of us all .
	manualset3
167446	2	412768	7	NULL	NULL	0	NULL	good 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The tension must be maintained for the good of us all .
	manualset3
167447	3	412768	7	NULL	NULL	0	NULL	all	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The tension must be maintained for the good of us all .
	manualset3
167448	1	412769	7	NULL	NULL	0	NULL	 term	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The term incretin effect was used to describe the fact that oral glucose load produces a greater insulin response than that of an isoglycemic intravenous glucose infusion .
	manualset3
167449	2	412769	7	NULL	NULL	0	NULL	incretin effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The term incretin effect was used to describe the fact that oral glucose load produces a greater insulin response than that of an isoglycemic intravenous glucose infusion .
	manualset3
167450	3	412769	7	NULL	NULL	NULL	NULL	oral glucose load	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The term incretin effect was used to describe the fact that oral glucose load produces a greater insulin response than that of an isoglycemic intravenous glucose infusion .
	manualset3
167451	4	412769	7	NULL	NULL	0	NULL	 insulin response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The term incretin effect was used to describe the fact that oral glucose load produces a greater insulin response than that of an isoglycemic intravenous glucose infusion .
	manualset3
167452	5	412769	7	NULL	NULL	0	NULL	isoglycemic intravenous glucose infusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The term incretin effect was used to describe the fact that oral glucose load produces a greater insulin response than that of an isoglycemic intravenous glucose infusion .
	manualset3
173652	6	412769	7	NULL	NULL	0	NULL	fact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The term incretin effect was used to describe the fact that oral glucose load produces a greater insulin response than that of an isoglycemic intravenous glucose infusion .
	manualset3
167453	1	412770	7	NULL	NULL	NULL	NULL	term	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The term minimally invasive cardiac surgery encompasses a number of different techniques , each with its own rationale , origin , and development , but all focusing on limiting the physiologic trespass of cardiac surgery on the patient .
	manualset3
167454	2	412770	7	NULL	NULL	0	NULL	minimally invasive cardiac surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The term minimally invasive cardiac surgery encompasses a number of different techniques , each with its own rationale , origin , and development , but all focusing on limiting the physiologic trespass of cardiac surgery on the patient .
	manualset3
167455	3	412770	7	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The term minimally invasive cardiac surgery encompasses a number of different techniques , each with its own rationale , origin , and development , but all focusing on limiting the physiologic trespass of cardiac surgery on the patient .
	manualset3
167456	4	412770	7	NULL	NULL	0	NULL	different techniques	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The term minimally invasive cardiac surgery encompasses a number of different techniques , each with its own rationale , origin , and development , but all focusing on limiting the physiologic trespass of cardiac surgery on the patient .
	manualset3
167457	5	412770	7	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The term minimally invasive cardiac surgery encompasses a number of different techniques , each with its own rationale , origin , and development , but all focusing on limiting the physiologic trespass of cardiac surgery on the patient .
	manualset3
167458	6	412770	7	NULL	NULL	0	NULL	physiologic trespass	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The term minimally invasive cardiac surgery encompasses a number of different techniques , each with its own rationale , origin , and development , but all focusing on limiting the physiologic trespass of cardiac surgery on the patient .
	manualset3
167459	7	412770	7	NULL	NULL	0	NULL	cardiac surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The term minimally invasive cardiac surgery encompasses a number of different techniques , each with its own rationale , origin , and development , but all focusing on limiting the physiologic trespass of cardiac surgery on the patient .
	manualset3
167460	8	412770	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The term minimally invasive cardiac surgery encompasses a number of different techniques , each with its own rationale , origin , and development , but all focusing on limiting the physiologic trespass of cardiac surgery on the patient .
	manualset3
167461	1	412771	7	NULL	NULL	0	NULL	term	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The term unstable angina should only be used to describe patients whose immediate prognosis is uncertain and the nature of the unstable disease may vary on a patient to patient basis , making broad categorization of such patients inappropriate .
	manualset3
167462	2	412771	7	NULL	NULL	0	NULL	unstable angina	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The term unstable angina should only be used to describe patients whose immediate prognosis is uncertain and the nature of the unstable disease may vary on a patient to patient basis , making broad categorization of such patients inappropriate .
	manualset3
167463	3	412771	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The term unstable angina should only be used to describe patients whose immediate prognosis is uncertain and the nature of the unstable disease may vary on a patient to patient basis , making broad categorization of such patients inappropriate .
	manualset3
167464	4	412771	7	NULL	NULL	0	NULL	prognosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The term unstable angina should only be used to describe patients whose immediate prognosis is uncertain and the nature of the unstable disease may vary on a patient to patient basis , making broad categorization of such patients inappropriate .
	manualset3
167465	5	412771	7	NULL	NULL	0	NULL	nature	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The term unstable angina should only be used to describe patients whose immediate prognosis is uncertain and the nature of the unstable disease may vary on a patient to patient basis , making broad categorization of such patients inappropriate .
	manualset3
167466	6	412771	7	NULL	NULL	0	NULL	unstable disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The term unstable angina should only be used to describe patients whose immediate prognosis is uncertain and the nature of the unstable disease may vary on a patient to patient basis , making broad categorization of such patients inappropriate .
	manualset3
167467	7	412771	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The term unstable angina should only be used to describe patients whose immediate prognosis is uncertain and the nature of the unstable disease may vary on a patient to patient basis , making broad categorization of such patients inappropriate .
	manualset3
167468	8	412771	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The term unstable angina should only be used to describe patients whose immediate prognosis is uncertain and the nature of the unstable disease may vary on a patient to patient basis , making broad categorization of such patients inappropriate .
	manualset3
167469	9	412771	7	NULL	NULL	0	NULL	broad categorization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The term unstable angina should only be used to describe patients whose immediate prognosis is uncertain and the nature of the unstable disease may vary on a patient to patient basis , making broad categorization of such patients inappropriate .
	manualset3
167470	10	412771	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The term unstable angina should only be used to describe patients whose immediate prognosis is uncertain and the nature of the unstable disease may vary on a patient to patient basis , making broad categorization of such patients inappropriate .
	manualset3
167471	1	412772	7	NULL	NULL	0	NULL	terminal bronchioles 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The terminal bronchioles and their short respiratory bronchioles inthe NO2-exposed animals developed stenosis , which increased with time .
	manualset3
167472	2	412772	7	NULL	NULL	0	NULL	short respiratory bronchioles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The terminal bronchioles and their short respiratory bronchioles inthe NO2-exposed animals developed stenosis , which increased with time .
	manualset3
167473	3	412772	7	NULL	NULL	0	NULL	NO2-exposed animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The terminal bronchioles and their short respiratory bronchioles inthe NO2-exposed animals developed stenosis , which increased with time .
	manualset3
167474	4	412772	7	NULL	NULL	0	NULL	stenosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The terminal bronchioles and their short respiratory bronchioles inthe NO2-exposed animals developed stenosis , which increased with time .
	manualset3
167475	5	412772	7	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The terminal bronchioles and their short respiratory bronchioles inthe NO2-exposed animals developed stenosis , which increased with time .
	manualset3
167476	1	412773	7	NULL	NULL	0	NULL	terminal field 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The terminal field of NL occupies a discrete zone in the rostromedial portion of the contralateral ICc , which we have termed the `` core '' of ICc .
	manualset3
167477	2	412773	7	NULL	NULL	0	NULL	NL	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The terminal field of NL occupies a discrete zone in the rostromedial portion of the contralateral ICc , which we have termed the `` core '' of ICc .
	manualset3
167478	3	412773	7	NULL	NULL	0	NULL	discrete zone	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The terminal field of NL occupies a discrete zone in the rostromedial portion of the contralateral ICc , which we have termed the `` core '' of ICc .
	manualset3
167479	4	412773	7	NULL	NULL	0	NULL	rostromedial portion	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The terminal field of NL occupies a discrete zone in the rostromedial portion of the contralateral ICc , which we have termed the `` core '' of ICc .
	manualset3
167480	5	412773	7	NULL	NULL	0	NULL	contralateral ICc	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The terminal field of NL occupies a discrete zone in the rostromedial portion of the contralateral ICc , which we have termed the `` core '' of ICc .
	manualset3
167481	6	412773	7	NULL	NULL	0	NULL	`` core ''	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The terminal field of NL occupies a discrete zone in the rostromedial portion of the contralateral ICc , which we have termed the `` core '' of ICc .
	manualset3
167482	7	412773	7	NULL	NULL	0	NULL	ICc	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The terminal field of NL occupies a discrete zone in the rostromedial portion of the contralateral ICc , which we have termed the `` core '' of ICc .
	manualset3
167483	1	412774	7	NULL	NULL	0	NULL	 terminal sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The terminal sequences of transcripts obtained by 3 ' rapid amplification of cDNA ends demonstrated the presence of polyadenylation .
	manualset3
167484	2	412774	7	NULL	NULL	0	NULL	 transcripts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The terminal sequences of transcripts obtained by 3 ' rapid amplification of cDNA ends demonstrated the presence of polyadenylation .
	manualset3
167485	3	412774	7	NULL	NULL	0	NULL	3 ' rapid amplification 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The terminal sequences of transcripts obtained by 3 ' rapid amplification of cDNA ends demonstrated the presence of polyadenylation .
	manualset3
167486	4	412774	7	NULL	NULL	NULL	NULL	cDNA ends	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The terminal sequences of transcripts obtained by 3 ' rapid amplification of cDNA ends demonstrated the presence of polyadenylation .
	manualset3
167487	5	412774	7	NULL	NULL	0	NULL	presence 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The terminal sequences of transcripts obtained by 3 ' rapid amplification of cDNA ends demonstrated the presence of polyadenylation .
	manualset3
167488	6	412774	7	NULL	NULL	0	NULL	polyadenylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The terminal sequences of transcripts obtained by 3 ' rapid amplification of cDNA ends demonstrated the presence of polyadenylation .
	manualset3
167489	1	412775	7	NULL	NULL	0	NULL	 test chart 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The test chart consists of a white tangent screen with 23 numbered fixation points located eccentrically at strategic points in relation to a central black spot , which is the test stimulus .
	manualset3
167490	2	412775	7	NULL	NULL	0	NULL	 white tangent screen	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The test chart consists of a white tangent screen with 23 numbered fixation points located eccentrically at strategic points in relation to a central black spot , which is the test stimulus .
	manualset3
167491	3	412775	7	NULL	NULL	NULL	NULL	23 numbered fixation points	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The test chart consists of a white tangent screen with 23 numbered fixation points located eccentrically at strategic points in relation to a central black spot , which is the test stimulus .
	manualset3
167492	4	412775	7	NULL	NULL	NULL	NULL	strategic points	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The test chart consists of a white tangent screen with 23 numbered fixation points located eccentrically at strategic points in relation to a central black spot , which is the test stimulus .
	manualset3
167493	5	412775	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The test chart consists of a white tangent screen with 23 numbered fixation points located eccentrically at strategic points in relation to a central black spot , which is the test stimulus .
	manualset3
167494	6	412775	7	NULL	NULL	0	NULL	central black spot	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The test chart consists of a white tangent screen with 23 numbered fixation points located eccentrically at strategic points in relation to a central black spot , which is the test stimulus .
	manualset3
167495	7	412775	7	NULL	NULL	NULL	NULL	test stimulus	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The test chart consists of a white tangent screen with 23 numbered fixation points located eccentrically at strategic points in relation to a central black spot , which is the test stimulus .
	manualset3
167496	1	412776	7	NULL	NULL	NULL	NULL	test results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The test results show that the consistency of eye drop preparations and their resulting physical-chemical properties like viscosity influence the quantity of the maximal force during the drop impact .
	manualset3
167497	2	412776	7	NULL	NULL	0	NULL	consistency	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The test results show that the consistency of eye drop preparations and their resulting physical-chemical properties like viscosity influence the quantity of the maximal force during the drop impact .
	manualset3
167498	3	412776	7	NULL	NULL	NULL	NULL	eye drop preparations	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The test results show that the consistency of eye drop preparations and their resulting physical-chemical properties like viscosity influence the quantity of the maximal force during the drop impact .
	manualset3
167499	4	412776	7	NULL	NULL	NULL	NULL	physical-chemical properties	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The test results show that the consistency of eye drop preparations and their resulting physical-chemical properties like viscosity influence the quantity of the maximal force during the drop impact .
	manualset3
167500	5	412776	7	NULL	NULL	0	NULL	viscosity 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The test results show that the consistency of eye drop preparations and their resulting physical-chemical properties like viscosity influence the quantity of the maximal force during the drop impact .
	manualset3
167501	6	412776	7	NULL	NULL	0	NULL	 quantity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The test results show that the consistency of eye drop preparations and their resulting physical-chemical properties like viscosity influence the quantity of the maximal force during the drop impact .
	manualset3
167502	7	412776	7	NULL	NULL	0	NULL	 maximal force	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The test results show that the consistency of eye drop preparations and their resulting physical-chemical properties like viscosity influence the quantity of the maximal force during the drop impact .
	manualset3
167503	8	412776	7	NULL	NULL	NULL	NULL	 drop impact	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The test results show that the consistency of eye drop preparations and their resulting physical-chemical properties like viscosity influence the quantity of the maximal force during the drop impact .
	manualset3
167504	1	412777	7	NULL	NULL	0	NULL	 test strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The test strains multiplied in both bacterial growth medium and commercial infant-feeding formula controls , with the exception of the Campylobacter strains , which were markedly inhibited in formula .
	manualset3
167505	2	412777	7	NULL	NULL	NULL	NULL	bacterial growth medium	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The test strains multiplied in both bacterial growth medium and commercial infant-feeding formula controls , with the exception of the Campylobacter strains , which were markedly inhibited in formula .
	manualset3
167506	3	412777	7	NULL	NULL	0	NULL	commercial infant-feeding formula controls	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The test strains multiplied in both bacterial growth medium and commercial infant-feeding formula controls , with the exception of the Campylobacter strains , which were markedly inhibited in formula .
	manualset3
167507	4	412777	7	NULL	NULL	0	NULL	exception	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The test strains multiplied in both bacterial growth medium and commercial infant-feeding formula controls , with the exception of the Campylobacter strains , which were markedly inhibited in formula .
	manualset3
167508	5	412777	7	NULL	NULL	0	NULL	Campylobacter strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The test strains multiplied in both bacterial growth medium and commercial infant-feeding formula controls , with the exception of the Campylobacter strains , which were markedly inhibited in formula .
	manualset3
167509	6	412777	7	NULL	NULL	NULL	NULL	formula	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The test strains multiplied in both bacterial growth medium and commercial infant-feeding formula controls , with the exception of the Campylobacter strains , which were markedly inhibited in formula .
	manualset3
167510	1	412778	7	NULL	NULL	0	NULL	Achievement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Achievement of feeding milestones after primary repair of long-gap esophageal atresia .
	manualset3
167511	2	412778	7	NULL	NULL	0	NULL	feeding milestones	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Achievement of feeding milestones after primary repair of long-gap esophageal atresia .
	manualset3
167512	3	412778	7	NULL	NULL	0	NULL	primary repair	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Achievement of feeding milestones after primary repair of long-gap esophageal atresia .
	manualset3
167513	4	412778	7	NULL	NULL	0	NULL	long-gap esophageal atresia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Achievement of feeding milestones after primary repair of long-gap esophageal atresia .
	manualset3
167514	1	412779	7	NULL	NULL	0	NULL	testing design	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The testing design assessed the reaction of fostered animals to a novel species ( M. pinetorum ) as well as to the parental and biological species .
	manualset3
167515	2	412779	7	NULL	NULL	0	NULL	reaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The testing design assessed the reaction of fostered animals to a novel species ( M. pinetorum ) as well as to the parental and biological species .
	manualset3
167516	3	412779	7	NULL	NULL	0	NULL	fostered animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The testing design assessed the reaction of fostered animals to a novel species ( M. pinetorum ) as well as to the parental and biological species .
	manualset3
167517	4	412779	7	NULL	NULL	0	NULL	novel species ( M. pinetorum )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The testing design assessed the reaction of fostered animals to a novel species ( M. pinetorum ) as well as to the parental and biological species .
	manualset3
167518	5	412779	7	NULL	NULL	0	NULL	parental species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The testing design assessed the reaction of fostered animals to a novel species ( M. pinetorum ) as well as to the parental and biological species .
	manualset3
167519	6	412779	7	NULL	NULL	0	NULL	biological species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The testing design assessed the reaction of fostered animals to a novel species ( M. pinetorum ) as well as to the parental and biological species .
	manualset3
167520	1	412780	7	NULL	NULL	0	NULL	tetra-carboxyl-ate ligand mol-ecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The tetra-carboxyl-ate ligand mol-ecules connect the Zn ( II ) atoms , completing a three-dimensional metal-organic framework .
	manualset3
167521	2	412780	7	NULL	NULL	0	NULL	Zn ( II ) atoms	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The tetra-carboxyl-ate ligand mol-ecules connect the Zn ( II ) atoms , completing a three-dimensional metal-organic framework .
	manualset3
167522	3	412780	7	NULL	NULL	0	NULL	three-dimensional metal-organic framework	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The tetra-carboxyl-ate ligand mol-ecules connect the Zn ( II ) atoms , completing a three-dimensional metal-organic framework .
	manualset3
167523	1	412781	7	NULL	NULL	0	NULL	 tetramer	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The tetramer dissociates into a dimer as demonstrated by a decreasing sedimentation coefficient with decreasing protein concentration .
	manualset3
167524	2	412781	7	NULL	NULL	0	NULL	dimer	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The tetramer dissociates into a dimer as demonstrated by a decreasing sedimentation coefficient with decreasing protein concentration .
	manualset3
167525	3	412781	7	NULL	NULL	0	NULL	decreasing sedimentation coefficient	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The tetramer dissociates into a dimer as demonstrated by a decreasing sedimentation coefficient with decreasing protein concentration .
	manualset3
167526	4	412781	7	NULL	NULL	0	NULL	decreasing protein concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The tetramer dissociates into a dimer as demonstrated by a decreasing sedimentation coefficient with decreasing protein concentration .
	manualset3
167527	1	412782	7	NULL	NULL	0	NULL	 theoretical possibility	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The theoretical possibility of improving renal function by administration of certain amino acids ( Arginine and Glycine ) , is not confirmed in practice , possibly due to the incidence of oxidative stress .
	manualset3
167528	2	412782	7	NULL	NULL	0	NULL	renal function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The theoretical possibility of improving renal function by administration of certain amino acids ( Arginine and Glycine ) , is not confirmed in practice , possibly due to the incidence of oxidative stress .
	manualset3
167529	3	412782	7	NULL	NULL	0	NULL	administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The theoretical possibility of improving renal function by administration of certain amino acids ( Arginine and Glycine ) , is not confirmed in practice , possibly due to the incidence of oxidative stress .
	manualset3
167530	4	412782	7	NULL	NULL	0	NULL	amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The theoretical possibility of improving renal function by administration of certain amino acids ( Arginine and Glycine ) , is not confirmed in practice , possibly due to the incidence of oxidative stress .
	manualset3
167531	5	412782	7	NULL	NULL	0	NULL	Arginine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The theoretical possibility of improving renal function by administration of certain amino acids ( Arginine and Glycine ) , is not confirmed in practice , possibly due to the incidence of oxidative stress .
	manualset3
167532	6	412782	7	NULL	NULL	0	NULL	 Glycine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The theoretical possibility of improving renal function by administration of certain amino acids ( Arginine and Glycine ) , is not confirmed in practice , possibly due to the incidence of oxidative stress .
	manualset3
167533	7	412782	7	NULL	NULL	0	NULL	incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The theoretical possibility of improving renal function by administration of certain amino acids ( Arginine and Glycine ) , is not confirmed in practice , possibly due to the incidence of oxidative stress .
	manualset3
167534	8	412782	7	NULL	NULL	0	NULL	oxidative stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The theoretical possibility of improving renal function by administration of certain amino acids ( Arginine and Glycine ) , is not confirmed in practice , possibly due to the incidence of oxidative stress .
	manualset3
167535	1	412783	7	NULL	NULL	0	NULL	 therapeutic observance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The therapeutic observance is a real issue of chronic diseases .
	manualset3
167536	2	412783	7	NULL	NULL	0	NULL	real issue	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The therapeutic observance is a real issue of chronic diseases .
	manualset3
167537	3	412783	7	NULL	NULL	0	NULL	chronic diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The therapeutic observance is a real issue of chronic diseases .
	manualset3
167538	1	412784	7	NULL	NULL	0	NULL	therapeutic problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The therapeutic problems , including the future of the mother and of the child are discussed , insisting on the necessity of the chirurgical celerity in case of dystocia .
	manualset3
167539	2	412784	7	NULL	NULL	0	NULL	future	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The therapeutic problems , including the future of the mother and of the child are discussed , insisting on the necessity of the chirurgical celerity in case of dystocia .
	manualset3
167540	3	412784	7	NULL	NULL	0	NULL	mother	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The therapeutic problems , including the future of the mother and of the child are discussed , insisting on the necessity of the chirurgical celerity in case of dystocia .
	manualset3
167541	4	412784	7	NULL	NULL	0	NULL	 child 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The therapeutic problems , including the future of the mother and of the child are discussed , insisting on the necessity of the chirurgical celerity in case of dystocia .
	manualset3
167542	5	412784	7	NULL	NULL	0	NULL	chirurgical celerity	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The therapeutic problems , including the future of the mother and of the child are discussed , insisting on the necessity of the chirurgical celerity in case of dystocia .
	manualset3
167543	6	412784	7	NULL	NULL	0	NULL	dystocia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The therapeutic problems , including the future of the mother and of the child are discussed , insisting on the necessity of the chirurgical celerity in case of dystocia .
	manualset3
168349	7	412784	7	NULL	NULL	0	NULL	necessity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The therapeutic problems , including the future of the mother and of the child are discussed , insisting on the necessity of the chirurgical celerity in case of dystocia .
	manualset3
167544	1	412785	7	NULL	NULL	0	NULL	thermodynamics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The thermodynamics of translesion DNA synthesis past major adducts of enantiomeric analogs of antitumor Cisplatin .
	manualset3
167545	2	412785	7	NULL	NULL	0	NULL	translesion DNA synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The thermodynamics of translesion DNA synthesis past major adducts of enantiomeric analogs of antitumor Cisplatin .
	manualset3
167546	3	412785	7	NULL	NULL	0	NULL	enantiomeric analogs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The thermodynamics of translesion DNA synthesis past major adducts of enantiomeric analogs of antitumor Cisplatin .
	manualset3
167547	4	412785	7	NULL	NULL	0	NULL	antitumor Cisplatin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The thermodynamics of translesion DNA synthesis past major adducts of enantiomeric analogs of antitumor Cisplatin .
	manualset3
173653	5	412785	7	NULL	NULL	0	NULL	adducts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The thermodynamics of translesion DNA synthesis past major adducts of enantiomeric analogs of antitumor Cisplatin .
	manualset3
167548	1	412786	7	NULL	NULL	0	NULL	thiamine pyrophosphatase technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The thiamine pyrophosphatase technique as a indicator of morphology of the Golgi apparatus in the neurons .
	manualset3
167549	2	412786	7	NULL	NULL	0	NULL	 indicator	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The thiamine pyrophosphatase technique as a indicator of morphology of the Golgi apparatus in the neurons .
	manualset3
167550	3	412786	7	NULL	NULL	0	NULL	morphology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The thiamine pyrophosphatase technique as a indicator of morphology of the Golgi apparatus in the neurons .
	manualset3
167551	4	412786	7	NULL	NULL	0	NULL	Golgi apparatus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The thiamine pyrophosphatase technique as a indicator of morphology of the Golgi apparatus in the neurons .
	manualset3
167552	5	412786	7	NULL	NULL	0	NULL	neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The thiamine pyrophosphatase technique as a indicator of morphology of the Golgi apparatus in the neurons .
	manualset3
167553	1	412787	7	NULL	NULL	0	NULL	Achiral meteoritic amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Achiral meteoritic amino acids , glycine and alpha-methylalanine , with hydrogen isotope ( D/H ) chirality , acted as the source of chirality in asymmetric autocatalysis with amplification of ee to afford highly enantioenriched 5-pyrimidyl alkanols .
	manualset3
167554	2	412787	7	NULL	NULL	0	NULL	glycine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Achiral meteoritic amino acids , glycine and alpha-methylalanine , with hydrogen isotope ( D/H ) chirality , acted as the source of chirality in asymmetric autocatalysis with amplification of ee to afford highly enantioenriched 5-pyrimidyl alkanols .
	manualset3
167555	3	412787	7	NULL	NULL	0	NULL	alpha-methylalanine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Achiral meteoritic amino acids , glycine and alpha-methylalanine , with hydrogen isotope ( D/H ) chirality , acted as the source of chirality in asymmetric autocatalysis with amplification of ee to afford highly enantioenriched 5-pyrimidyl alkanols .
	manualset3
167556	4	412787	7	NULL	NULL	0	NULL	hydrogen isotope ( D/H ) chirality	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Achiral meteoritic amino acids , glycine and alpha-methylalanine , with hydrogen isotope ( D/H ) chirality , acted as the source of chirality in asymmetric autocatalysis with amplification of ee to afford highly enantioenriched 5-pyrimidyl alkanols .
	manualset3
167557	5	412787	7	NULL	NULL	NULL	NULL	 source	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Achiral meteoritic amino acids , glycine and alpha-methylalanine , with hydrogen isotope ( D/H ) chirality , acted as the source of chirality in asymmetric autocatalysis with amplification of ee to afford highly enantioenriched 5-pyrimidyl alkanols .
	manualset3
167558	6	412787	7	NULL	NULL	NULL	NULL	chirality 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Achiral meteoritic amino acids , glycine and alpha-methylalanine , with hydrogen isotope ( D/H ) chirality , acted as the source of chirality in asymmetric autocatalysis with amplification of ee to afford highly enantioenriched 5-pyrimidyl alkanols .
	manualset3
167559	7	412787	7	NULL	NULL	NULL	NULL	asymmetric autocatalysis	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Achiral meteoritic amino acids , glycine and alpha-methylalanine , with hydrogen isotope ( D/H ) chirality , acted as the source of chirality in asymmetric autocatalysis with amplification of ee to afford highly enantioenriched 5-pyrimidyl alkanols .
	manualset3
167560	8	412787	7	NULL	NULL	0	NULL	 amplification	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Achiral meteoritic amino acids , glycine and alpha-methylalanine , with hydrogen isotope ( D/H ) chirality , acted as the source of chirality in asymmetric autocatalysis with amplification of ee to afford highly enantioenriched 5-pyrimidyl alkanols .
	manualset3
167561	9	412787	7	NULL	NULL	0	NULL	ee 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Achiral meteoritic amino acids , glycine and alpha-methylalanine , with hydrogen isotope ( D/H ) chirality , acted as the source of chirality in asymmetric autocatalysis with amplification of ee to afford highly enantioenriched 5-pyrimidyl alkanols .
	manualset3
167562	10	412787	7	NULL	NULL	0	NULL	highly enantioenriched 5-pyrimidyl alkanols	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Achiral meteoritic amino acids , glycine and alpha-methylalanine , with hydrogen isotope ( D/H ) chirality , acted as the source of chirality in asymmetric autocatalysis with amplification of ee to afford highly enantioenriched 5-pyrimidyl alkanols .
	manualset3
167563	1	412788	7	NULL	NULL	0	NULL	 third case	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The third case , with a FOXL2 mutant allele imbalance , showed a diminished mutant allele population ( 32 % ) despite high estimated tumor content ( & gt ; 90 % ) , suggesting tumor heterogeneity for the mutation .
	manualset3
167564	2	412788	7	NULL	NULL	0	NULL	FOXL2 mutant allele imbalance	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The third case , with a FOXL2 mutant allele imbalance , showed a diminished mutant allele population ( 32 % ) despite high estimated tumor content ( & gt ; 90 % ) , suggesting tumor heterogeneity for the mutation .
	manualset3
167565	3	412788	7	NULL	NULL	0	NULL	mutant allele population 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The third case , with a FOXL2 mutant allele imbalance , showed a diminished mutant allele population ( 32 % ) despite high estimated tumor content ( & gt ; 90 % ) , suggesting tumor heterogeneity for the mutation .
	manualset3
167566	4	412788	7	NULL	NULL	0	NULL	32 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The third case , with a FOXL2 mutant allele imbalance , showed a diminished mutant allele population ( 32 % ) despite high estimated tumor content ( & gt ; 90 % ) , suggesting tumor heterogeneity for the mutation .
	manualset3
167567	5	412788	7	NULL	NULL	0	NULL	tumor content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The third case , with a FOXL2 mutant allele imbalance , showed a diminished mutant allele population ( 32 % ) despite high estimated tumor content ( & gt ; 90 % ) , suggesting tumor heterogeneity for the mutation .
	manualset3
167568	6	412788	7	NULL	NULL	0	NULL	& gt ; 90 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The third case , with a FOXL2 mutant allele imbalance , showed a diminished mutant allele population ( 32 % ) despite high estimated tumor content ( & gt ; 90 % ) , suggesting tumor heterogeneity for the mutation .
	manualset3
167569	7	412788	7	NULL	NULL	0	NULL	tumor heterogeneity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The third case , with a FOXL2 mutant allele imbalance , showed a diminished mutant allele population ( 32 % ) despite high estimated tumor content ( & gt ; 90 % ) , suggesting tumor heterogeneity for the mutation .
	manualset3
167570	8	412788	7	NULL	NULL	0	NULL	mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The third case , with a FOXL2 mutant allele imbalance , showed a diminished mutant allele population ( 32 % ) despite high estimated tumor content ( & gt ; 90 % ) , suggesting tumor heterogeneity for the mutation .
	manualset3
167571	1	412789	7	NULL	NULL	0	NULL	third component	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The third component of complement ( C3 ) bound to tumor target cells enhances their sensitivity to killing by activated macrophages .
	manualset3
167572	2	412789	7	NULL	NULL	0	NULL	complement ( C3 )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The third component of complement ( C3 ) bound to tumor target cells enhances their sensitivity to killing by activated macrophages .
	manualset3
167573	3	412789	7	NULL	NULL	0	NULL	tumor target cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The third component of complement ( C3 ) bound to tumor target cells enhances their sensitivity to killing by activated macrophages .
	manualset3
167574	4	412789	7	NULL	NULL	0	NULL	sensitivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The third component of complement ( C3 ) bound to tumor target cells enhances their sensitivity to killing by activated macrophages .
	manualset3
167575	5	412789	7	NULL	NULL	0	NULL	activated macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The third component of complement ( C3 ) bound to tumor target cells enhances their sensitivity to killing by activated macrophages .
	manualset3
167576	1	412790	7	NULL	NULL	0	NULL	third group	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The third group with a midline decompression and preservation of the articular processes had an added intertransverse process fusion between the olisthetic levels .
	manualset3
167577	2	412790	7	NULL	NULL	NULL	NULL	midline decompression	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The third group with a midline decompression and preservation of the articular processes had an added intertransverse process fusion between the olisthetic levels .
	manualset3
167578	3	412790	7	NULL	NULL	0	NULL	preservation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The third group with a midline decompression and preservation of the articular processes had an added intertransverse process fusion between the olisthetic levels .
	manualset3
167579	4	412790	7	NULL	NULL	0	NULL	 articular processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The third group with a midline decompression and preservation of the articular processes had an added intertransverse process fusion between the olisthetic levels .
	manualset3
167580	5	412790	7	NULL	NULL	0	NULL	intertransverse process fusion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The third group with a midline decompression and preservation of the articular processes had an added intertransverse process fusion between the olisthetic levels .
	manualset3
167581	6	412790	7	NULL	NULL	0	NULL	olisthetic levels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The third group with a midline decompression and preservation of the articular processes had an added intertransverse process fusion between the olisthetic levels .
	manualset3
167582	1	412791	7	NULL	NULL	0	NULL	 third pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The third pathway of the abnormal splicing revealed a rare class of transcript that has the last intron retained in the mature RNA .
	manualset3
167583	2	412791	7	NULL	NULL	0	NULL	abnormal splicing	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The third pathway of the abnormal splicing revealed a rare class of transcript that has the last intron retained in the mature RNA .
	manualset3
167584	3	412791	7	NULL	NULL	0	NULL	rare class	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The third pathway of the abnormal splicing revealed a rare class of transcript that has the last intron retained in the mature RNA .
	manualset3
167585	4	412791	7	NULL	NULL	0	NULL	transcript	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The third pathway of the abnormal splicing revealed a rare class of transcript that has the last intron retained in the mature RNA .
	manualset3
167586	5	412791	7	NULL	NULL	0	NULL	 last intron	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The third pathway of the abnormal splicing revealed a rare class of transcript that has the last intron retained in the mature RNA .
	manualset3
167587	6	412791	7	NULL	NULL	0	NULL	 mature RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The third pathway of the abnormal splicing revealed a rare class of transcript that has the last intron retained in the mature RNA .
	manualset3
167588	1	412792	7	NULL	NULL	0	NULL	 thoughts	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The thoughts on facilitation combine the use of recognized knowledge , experience and reflection to offer a way of reducing the risk of rejection of reflective practice .
	manualset3
167589	2	412792	7	NULL	NULL	0	NULL	facilitation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The thoughts on facilitation combine the use of recognized knowledge , experience and reflection to offer a way of reducing the risk of rejection of reflective practice .
	manualset3
167590	3	412792	7	NULL	NULL	0	NULL	recognized knowledge	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The thoughts on facilitation combine the use of recognized knowledge , experience and reflection to offer a way of reducing the risk of rejection of reflective practice .
	manualset3
167591	4	412792	7	NULL	NULL	NULL	NULL	 experience 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The thoughts on facilitation combine the use of recognized knowledge , experience and reflection to offer a way of reducing the risk of rejection of reflective practice .
	manualset3
167592	5	412792	7	NULL	NULL	0	NULL	reflection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The thoughts on facilitation combine the use of recognized knowledge , experience and reflection to offer a way of reducing the risk of rejection of reflective practice .
	manualset3
167593	6	412792	7	NULL	NULL	0	NULL	way	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The thoughts on facilitation combine the use of recognized knowledge , experience and reflection to offer a way of reducing the risk of rejection of reflective practice .
	manualset3
167594	7	412792	7	NULL	NULL	0	NULL	reducing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The thoughts on facilitation combine the use of recognized knowledge , experience and reflection to offer a way of reducing the risk of rejection of reflective practice .
	manualset3
167595	8	412792	7	NULL	NULL	0	NULL	risk of rejection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The thoughts on facilitation combine the use of recognized knowledge , experience and reflection to offer a way of reducing the risk of rejection of reflective practice .
	manualset3
167596	9	412792	7	NULL	NULL	NULL	NULL	reflective practice	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The thoughts on facilitation combine the use of recognized knowledge , experience and reflection to offer a way of reducing the risk of rejection of reflective practice .
	manualset3
167597	1	412793	7	NULL	NULL	0	NULL	 three B6 bipolar cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The three B6 bipolar cells studied made narrow-cleft , semi-invaginating basal junctions with cone pedicles .
	manualset3
167598	2	412793	7	NULL	NULL	0	NULL	narrow-cleft	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The three B6 bipolar cells studied made narrow-cleft , semi-invaginating basal junctions with cone pedicles .
	manualset3
167599	3	412793	7	NULL	NULL	0	NULL	semi-invaginating basal junctions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The three B6 bipolar cells studied made narrow-cleft , semi-invaginating basal junctions with cone pedicles .
	manualset3
167600	4	412793	7	NULL	NULL	0	NULL	cone pedicles	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The three B6 bipolar cells studied made narrow-cleft , semi-invaginating basal junctions with cone pedicles .
	manualset3
167601	1	412794	7	NULL	NULL	0	NULL	three forms	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The three forms showed similar protein accumulation in transgenic seeds ; however , only HaHSFA9-SRDX showed a highly significant reduction of seed longevity , as determined by controlled deterioration tests , a rapid seed ageing procedure .
	manualset3
167602	2	412794	7	NULL	NULL	0	NULL	protein accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The three forms showed similar protein accumulation in transgenic seeds ; however , only HaHSFA9-SRDX showed a highly significant reduction of seed longevity , as determined by controlled deterioration tests , a rapid seed ageing procedure .
	manualset3
167603	3	412794	7	NULL	NULL	0	NULL	transgenic seeds	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The three forms showed similar protein accumulation in transgenic seeds ; however , only HaHSFA9-SRDX showed a highly significant reduction of seed longevity , as determined by controlled deterioration tests , a rapid seed ageing procedure .
	manualset3
167604	4	412794	7	NULL	NULL	0	NULL	HaHSFA9-SRDX	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The three forms showed similar protein accumulation in transgenic seeds ; however , only HaHSFA9-SRDX showed a highly significant reduction of seed longevity , as determined by controlled deterioration tests , a rapid seed ageing procedure .
	manualset3
167605	5	412794	7	NULL	NULL	0	NULL	reduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The three forms showed similar protein accumulation in transgenic seeds ; however , only HaHSFA9-SRDX showed a highly significant reduction of seed longevity , as determined by controlled deterioration tests , a rapid seed ageing procedure .
	manualset3
167606	6	412794	7	NULL	NULL	NULL	NULL	seed longevity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The three forms showed similar protein accumulation in transgenic seeds ; however , only HaHSFA9-SRDX showed a highly significant reduction of seed longevity , as determined by controlled deterioration tests , a rapid seed ageing procedure .
	manualset3
167607	7	412794	7	NULL	NULL	NULL	NULL	controlled deterioration tests	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The three forms showed similar protein accumulation in transgenic seeds ; however , only HaHSFA9-SRDX showed a highly significant reduction of seed longevity , as determined by controlled deterioration tests , a rapid seed ageing procedure .
	manualset3
167608	8	412794	7	NULL	NULL	NULL	NULL	rapid seed ageing procedure	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The three forms showed similar protein accumulation in transgenic seeds ; however , only HaHSFA9-SRDX showed a highly significant reduction of seed longevity , as determined by controlled deterioration tests , a rapid seed ageing procedure .
	manualset3
167609	1	412795	7	NULL	NULL	0	NULL	three mitochondrial carrier family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The three mitochondrial carrier family characteristic intrahelical arginines are essential for nucleotide binding .
	manualset3
167610	2	412795	7	NULL	NULL	0	NULL	intrahelical arginines	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The three mitochondrial carrier family characteristic intrahelical arginines are essential for nucleotide binding .
	manualset3
167611	3	412795	7	NULL	NULL	0	NULL	nucleotide binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The three mitochondrial carrier family characteristic intrahelical arginines are essential for nucleotide binding .
	manualset3
167612	1	412796	7	NULL	NULL	0	NULL	Acid ingestion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acid ingestion , particularly with suicidal intent , is not a rare occurrence , and the radiologist has an important part in its diagnosis , evaluation and management .
	manualset3
167613	2	412796	7	NULL	NULL	0	NULL	suicidal intent	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acid ingestion , particularly with suicidal intent , is not a rare occurrence , and the radiologist has an important part in its diagnosis , evaluation and management .
	manualset3
167614	3	412796	7	NULL	NULL	0	NULL	occurrence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Acid ingestion , particularly with suicidal intent , is not a rare occurrence , and the radiologist has an important part in its diagnosis , evaluation and management .
	manualset3
167615	4	412796	7	NULL	NULL	0	NULL	 radiologist	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Acid ingestion , particularly with suicidal intent , is not a rare occurrence , and the radiologist has an important part in its diagnosis , evaluation and management .
	manualset3
167616	5	412796	7	NULL	NULL	0	NULL	part 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acid ingestion , particularly with suicidal intent , is not a rare occurrence , and the radiologist has an important part in its diagnosis , evaluation and management .
	manualset3
167617	6	412796	7	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acid ingestion , particularly with suicidal intent , is not a rare occurrence , and the radiologist has an important part in its diagnosis , evaluation and management .
	manualset3
167618	7	412796	7	NULL	NULL	0	NULL	evaluation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Acid ingestion , particularly with suicidal intent , is not a rare occurrence , and the radiologist has an important part in its diagnosis , evaluation and management .
	manualset3
167619	8	412796	7	NULL	NULL	0	NULL	management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Acid ingestion , particularly with suicidal intent , is not a rare occurrence , and the radiologist has an important part in its diagnosis , evaluation and management .
	manualset3
167620	1	412797	7	NULL	NULL	0	NULL	 three relatively stable hybridoma lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The three relatively stable hybridoma lines isolated secrete different Igs as judged by their antibody subclasses and differing abilities to inhibit HMG-CoA reductase in solution .
	manualset3
167621	2	412797	7	NULL	NULL	0	NULL	different Igs	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The three relatively stable hybridoma lines isolated secrete different Igs as judged by their antibody subclasses and differing abilities to inhibit HMG-CoA reductase in solution .
	manualset3
167622	3	412797	7	NULL	NULL	0	NULL	antibody subclasses	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The three relatively stable hybridoma lines isolated secrete different Igs as judged by their antibody subclasses and differing abilities to inhibit HMG-CoA reductase in solution .
	manualset3
167623	4	412797	7	NULL	NULL	0	NULL	abilities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The three relatively stable hybridoma lines isolated secrete different Igs as judged by their antibody subclasses and differing abilities to inhibit HMG-CoA reductase in solution .
	manualset3
167624	5	412797	7	NULL	NULL	0	NULL	HMG-CoA reductase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The three relatively stable hybridoma lines isolated secrete different Igs as judged by their antibody subclasses and differing abilities to inhibit HMG-CoA reductase in solution .
	manualset3
167625	6	412797	7	NULL	NULL	0	NULL	solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The three relatively stable hybridoma lines isolated secrete different Igs as judged by their antibody subclasses and differing abilities to inhibit HMG-CoA reductase in solution .
	manualset3
167626	1	412798	7	NULL	NULL	NULL	NULL	threshold remains	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The threshold remains yet to be established .
	manualset3
167627	1	412799	7	NULL	NULL	0	NULL	 thrombin time	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The thrombin time and anti-Xa test were only slightly influenced by concentrations up to 100 micrograms/mL .
	manualset3
167628	2	412799	7	NULL	NULL	0	NULL	anti-Xa test	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The thrombin time and anti-Xa test were only slightly influenced by concentrations up to 100 micrograms/mL .
	manualset3
167629	3	412799	7	NULL	NULL	0	NULL	concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The thrombin time and anti-Xa test were only slightly influenced by concentrations up to 100 micrograms/mL .
	manualset3
167630	4	412799	7	NULL	NULL	0	NULL	100 micrograms/mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The thrombin time and anti-Xa test were only slightly influenced by concentrations up to 100 micrograms/mL .
	manualset3
167631	1	412800	7	NULL	NULL	0	NULL	thymus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The thymus is practically devoid of Ig + cells in the embry and it is not clear whether there any Ig - + cells in the bone marrow .
	manualset3
167632	2	412800	7	NULL	NULL	0	NULL	Ig + cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The thymus is practically devoid of Ig + cells in the embry and it is not clear whether there any Ig - + cells in the bone marrow .
	manualset3
167633	3	412800	7	NULL	NULL	0	NULL	embry	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The thymus is practically devoid of Ig + cells in the embry and it is not clear whether there any Ig - + cells in the bone marrow .
	manualset3
167634	4	412800	7	NULL	NULL	0	NULL	Ig - + cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The thymus is practically devoid of Ig + cells in the embry and it is not clear whether there any Ig - + cells in the bone marrow .
	manualset3
167635	5	412800	7	NULL	NULL	0	NULL	bone marrow	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The thymus is practically devoid of Ig + cells in the embry and it is not clear whether there any Ig - + cells in the bone marrow .
	manualset3
167636	1	412801	7	NULL	NULL	0	NULL	thymus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The thymus of the homozygous nude mouse embryo is laid down normally .
	manualset3
167637	2	412801	7	NULL	NULL	0	NULL	homozygous nude mouse embryo	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The thymus of the homozygous nude mouse embryo is laid down normally .
	manualset3
167638	1	412802	7	NULL	NULL	0	NULL	thymus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The thymus plays a major role in myasthenia gravis ( MG ) .
	manualset3
167639	2	412802	7	NULL	NULL	0	NULL	major role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The thymus plays a major role in myasthenia gravis ( MG ) .
	manualset3
167640	3	412802	7	NULL	NULL	0	NULL	myasthenia gravis ( MG )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The thymus plays a major role in myasthenia gravis ( MG ) .
	manualset3
167641	1	412803	7	NULL	NULL	0	NULL	tick receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The tick receptor for outer surface protein A ( TROSPA ) is an Ixodes scapularis ( I. scapularis ) receptor for Borrelia burgdorferi ( B. burgdorferi ) , the causative agent of Lyme disease in North America .
	manualset3
167642	2	412803	7	NULL	NULL	0	NULL	outer surface protein A ( TROSPA )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The tick receptor for outer surface protein A ( TROSPA ) is an Ixodes scapularis ( I. scapularis ) receptor for Borrelia burgdorferi ( B. burgdorferi ) , the causative agent of Lyme disease in North America .
	manualset3
167643	3	412803	7	NULL	NULL	0	NULL	Ixodes scapularis ( I. scapularis ) receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The tick receptor for outer surface protein A ( TROSPA ) is an Ixodes scapularis ( I. scapularis ) receptor for Borrelia burgdorferi ( B. burgdorferi ) , the causative agent of Lyme disease in North America .
	manualset3
167644	4	412803	7	NULL	NULL	0	NULL	Borrelia burgdorferi ( B. burgdorferi )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The tick receptor for outer surface protein A ( TROSPA ) is an Ixodes scapularis ( I. scapularis ) receptor for Borrelia burgdorferi ( B. burgdorferi ) , the causative agent of Lyme disease in North America .
	manualset3
167645	5	412803	7	NULL	NULL	0	NULL	causative agent	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The tick receptor for outer surface protein A ( TROSPA ) is an Ixodes scapularis ( I. scapularis ) receptor for Borrelia burgdorferi ( B. burgdorferi ) , the causative agent of Lyme disease in North America .
	manualset3
167646	6	412803	7	NULL	NULL	0	NULL	Lyme disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The tick receptor for outer surface protein A ( TROSPA ) is an Ixodes scapularis ( I. scapularis ) receptor for Borrelia burgdorferi ( B. burgdorferi ) , the causative agent of Lyme disease in North America .
	manualset3
167647	7	412803	7	NULL	NULL	0	NULL	North America	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The tick receptor for outer surface protein A ( TROSPA ) is an Ixodes scapularis ( I. scapularis ) receptor for Borrelia burgdorferi ( B. burgdorferi ) , the causative agent of Lyme disease in North America .
	manualset3
167648	1	412804	7	NULL	NULL	0	NULL	time course	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The time course of collagenase inhibitor accumulation in blister fluid was studied using heat - and suction-induced bullae .
	manualset3
167649	2	412804	7	NULL	NULL	0	NULL	collagenase inhibitor accumulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The time course of collagenase inhibitor accumulation in blister fluid was studied using heat - and suction-induced bullae .
	manualset3
167650	3	412804	7	NULL	NULL	NULL	NULL	blister fluid	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The time course of collagenase inhibitor accumulation in blister fluid was studied using heat - and suction-induced bullae .
	manualset3
167651	4	412804	7	NULL	NULL	NULL	NULL	heat -induced bullae	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The time course of collagenase inhibitor accumulation in blister fluid was studied using heat - and suction-induced bullae .
	manualset3
167652	5	412804	7	NULL	NULL	NULL	NULL	suction-induced bullae	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The time course of collagenase inhibitor accumulation in blister fluid was studied using heat - and suction-induced bullae .
	manualset3
167653	1	412805	7	NULL	NULL	0	NULL	Acid phosphatase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acid phosphatase activity in microfilariae of Setaria labiato-papillosa and comparison with other blood microfilariae of dog and horse origin .
	manualset3
167654	2	412805	7	NULL	NULL	0	NULL	microfilariae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Acid phosphatase activity in microfilariae of Setaria labiato-papillosa and comparison with other blood microfilariae of dog and horse origin .
	manualset3
167655	3	412805	7	NULL	NULL	0	NULL	Setaria labiato-papillosa	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Acid phosphatase activity in microfilariae of Setaria labiato-papillosa and comparison with other blood microfilariae of dog and horse origin .
	manualset3
167656	4	412805	7	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Acid phosphatase activity in microfilariae of Setaria labiato-papillosa and comparison with other blood microfilariae of dog and horse origin .
	manualset3
167657	5	412805	7	NULL	NULL	0	NULL	blood microfilariae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Acid phosphatase activity in microfilariae of Setaria labiato-papillosa and comparison with other blood microfilariae of dog and horse origin .
	manualset3
167658	6	412805	7	NULL	NULL	0	NULL	dog	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Acid phosphatase activity in microfilariae of Setaria labiato-papillosa and comparison with other blood microfilariae of dog and horse origin .
	manualset3
167659	7	412805	7	NULL	NULL	0	NULL	horse	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Acid phosphatase activity in microfilariae of Setaria labiato-papillosa and comparison with other blood microfilariae of dog and horse origin .
	manualset3
167661	1	412806	7	NULL	NULL	0	NULL	 time course	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The time course of effects upon thermal denaturation indicated a rapid initial binding phase followed by a slower phase consistent with the stepwise cross-linking of DNA observed for a difunctional agent .
	manualset3
167662	2	412806	7	NULL	NULL	0	NULL	effects 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The time course of effects upon thermal denaturation indicated a rapid initial binding phase followed by a slower phase consistent with the stepwise cross-linking of DNA observed for a difunctional agent .
	manualset3
167663	3	412806	7	NULL	NULL	0	NULL	 thermal denaturation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The time course of effects upon thermal denaturation indicated a rapid initial binding phase followed by a slower phase consistent with the stepwise cross-linking of DNA observed for a difunctional agent .
	manualset3
167664	4	412806	7	NULL	NULL	0	NULL	rapid initial binding phase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The time course of effects upon thermal denaturation indicated a rapid initial binding phase followed by a slower phase consistent with the stepwise cross-linking of DNA observed for a difunctional agent .
	manualset3
167665	5	412806	7	NULL	NULL	0	NULL	slower phase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The time course of effects upon thermal denaturation indicated a rapid initial binding phase followed by a slower phase consistent with the stepwise cross-linking of DNA observed for a difunctional agent .
	manualset3
167666	6	412806	7	NULL	NULL	NULL	NULL	cross-linking	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The time course of effects upon thermal denaturation indicated a rapid initial binding phase followed by a slower phase consistent with the stepwise cross-linking of DNA observed for a difunctional agent .
	manualset3
167667	7	412806	7	NULL	NULL	0	NULL	difunctional agent 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The time course of effects upon thermal denaturation indicated a rapid initial binding phase followed by a slower phase consistent with the stepwise cross-linking of DNA observed for a difunctional agent .
	manualset3
167668	8	412806	7	NULL	NULL	NULL	NULL	stepwise  cross-linking	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The time course of effects upon thermal denaturation indicated a rapid initial binding phase followed by a slower phase consistent with the stepwise cross-linking of DNA observed for a difunctional agent .
	manualset3
168350	9	412806	7	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The time course of effects upon thermal denaturation indicated a rapid initial binding phase followed by a slower phase consistent with the stepwise cross-linking of DNA observed for a difunctional agent .
	manualset3
173654	10	412806	7	NULL	NULL	0	NULL	difunctional agent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The time course of effects upon thermal denaturation indicated a rapid initial binding phase followed by a slower phase consistent with the stepwise cross-linking of DNA observed for a difunctional agent .
	manualset3
167669	1	412807	7	NULL	NULL	0	NULL	 time course	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The time course of hERG channel deactivation was slowed at multiple potentials ( -120 to -70 mV ) .
	manualset3
167670	2	412807	7	NULL	NULL	0	NULL	hERG channel deactivation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The time course of hERG channel deactivation was slowed at multiple potentials ( -120 to -70 mV ) .
	manualset3
167671	3	412807	7	NULL	NULL	0	NULL	multiple potentials 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The time course of hERG channel deactivation was slowed at multiple potentials ( -120 to -70 mV ) .
	manualset3
167672	4	412807	7	NULL	NULL	0	NULL	-120 to -70 mV	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The time course of hERG channel deactivation was slowed at multiple potentials ( -120 to -70 mV ) .
	manualset3
167673	1	412808	7	NULL	NULL	0	NULL	time history	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The time history of quasi-static slip along the plate interface , based on small repeating earthquakes that were part of the migrating seismicity , suggests that two sequences involved slow-slip transients propagating toward the initial rupture point .
	manualset3
167674	2	412808	7	NULL	NULL	0	NULL	quasi-static slip	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The time history of quasi-static slip along the plate interface , based on small repeating earthquakes that were part of the migrating seismicity , suggests that two sequences involved slow-slip transients propagating toward the initial rupture point .
	manualset3
167675	3	412808	7	NULL	NULL	0	NULL	plate interface	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The time history of quasi-static slip along the plate interface , based on small repeating earthquakes that were part of the migrating seismicity , suggests that two sequences involved slow-slip transients propagating toward the initial rupture point .
	manualset3
167676	4	412808	7	NULL	NULL	0	NULL	small repeating earthquakes	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The time history of quasi-static slip along the plate interface , based on small repeating earthquakes that were part of the migrating seismicity , suggests that two sequences involved slow-slip transients propagating toward the initial rupture point .
	manualset3
167677	5	412808	7	NULL	NULL	NULL	NULL	migrating seismicity	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The time history of quasi-static slip along the plate interface , based on small repeating earthquakes that were part of the migrating seismicity , suggests that two sequences involved slow-slip transients propagating toward the initial rupture point .
	manualset3
167678	6	412808	7	NULL	NULL	0	NULL	two sequences	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The time history of quasi-static slip along the plate interface , based on small repeating earthquakes that were part of the migrating seismicity , suggests that two sequences involved slow-slip transients propagating toward the initial rupture point .
	manualset3
167679	7	412808	7	NULL	NULL	0	NULL	slow-slip transients	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The time history of quasi-static slip along the plate interface , based on small repeating earthquakes that were part of the migrating seismicity , suggests that two sequences involved slow-slip transients propagating toward the initial rupture point .
	manualset3
167680	8	412808	7	NULL	NULL	0	NULL	 initial rupture point	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The time history of quasi-static slip along the plate interface , based on small repeating earthquakes that were part of the migrating seismicity , suggests that two sequences involved slow-slip transients propagating toward the initial rupture point .
	manualset3
167681	1	412809	7	NULL	NULL	NULL	NULL	timely regulation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The timely regulation of gonadotropin-releasing hormone ( GnRH ) secretion requires a GABAergic signal .
	manualset3
167682	2	412809	7	NULL	NULL	0	NULL	gonadotropin-releasing hormone ( GnRH ) secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The timely regulation of gonadotropin-releasing hormone ( GnRH ) secretion requires a GABAergic signal .
	manualset3
167683	3	412809	7	NULL	NULL	0	NULL	GABAergic signal	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The timely regulation of gonadotropin-releasing hormone ( GnRH ) secretion requires a GABAergic signal .
	manualset3
167684	1	412810	7	NULL	NULL	0	NULL	timing 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The timing of hb expression in neuroblasts is regulated at the transcriptional level .
	manualset3
167685	2	412810	7	NULL	NULL	0	NULL	hb expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The timing of hb expression in neuroblasts is regulated at the transcriptional level .
	manualset3
167686	3	412810	7	NULL	NULL	0	NULL	neuroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The timing of hb expression in neuroblasts is regulated at the transcriptional level .
	manualset3
167687	4	412810	7	NULL	NULL	0	NULL	transcriptional level	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The timing of hb expression in neuroblasts is regulated at the transcriptional level .
	manualset3
167688	1	412811	7	NULL	NULL	0	NULL	tissue distribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The tissue distribution , pharmacokinetics , excretion and safety study were persuasive for the potential application of NOSC as a new drug carrier .
	manualset3
167689	2	412811	7	NULL	NULL	0	NULL	pharmacokinetics	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The tissue distribution , pharmacokinetics , excretion and safety study were persuasive for the potential application of NOSC as a new drug carrier .
	manualset3
167690	3	412811	7	NULL	NULL	0	NULL	excretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The tissue distribution , pharmacokinetics , excretion and safety study were persuasive for the potential application of NOSC as a new drug carrier .
	manualset3
167691	4	412811	7	NULL	NULL	0	NULL	safety study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The tissue distribution , pharmacokinetics , excretion and safety study were persuasive for the potential application of NOSC as a new drug carrier .
	manualset3
167692	5	412811	7	NULL	NULL	0	NULL	potential application	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The tissue distribution , pharmacokinetics , excretion and safety study were persuasive for the potential application of NOSC as a new drug carrier .
	manualset3
167693	6	412811	7	NULL	NULL	0	NULL	NOSC	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The tissue distribution , pharmacokinetics , excretion and safety study were persuasive for the potential application of NOSC as a new drug carrier .
	manualset3
167694	7	412811	7	NULL	NULL	NULL	NULL	 new drug carrier	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The tissue distribution , pharmacokinetics , excretion and safety study were persuasive for the potential application of NOSC as a new drug carrier .
	manualset3
167695	1	412812	7	NULL	NULL	0	NULL	tissue distribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The tissue distribution of P-glycoprotein ( Pgp ) and the structurally related cystic fibrosis transmembrane conductance regulator ( CFTR ) is apparently mutually exclusive , particularly in epithelial ; where one protein is expressed the other is not .
	manualset3
167696	2	412812	7	NULL	NULL	0	NULL	P-glycoprotein ( Pgp )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The tissue distribution of P-glycoprotein ( Pgp ) and the structurally related cystic fibrosis transmembrane conductance regulator ( CFTR ) is apparently mutually exclusive , particularly in epithelial ; where one protein is expressed the other is not .
	manualset3
167697	3	412812	7	NULL	NULL	0	NULL	cystic fibrosis transmembrane conductance regulator ( CFTR ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The tissue distribution of P-glycoprotein ( Pgp ) and the structurally related cystic fibrosis transmembrane conductance regulator ( CFTR ) is apparently mutually exclusive , particularly in epithelial ; where one protein is expressed the other is not .
	manualset3
167698	5	412812	7	NULL	NULL	NULL	NULL	one protein 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The tissue distribution of P-glycoprotein ( Pgp ) and the structurally related cystic fibrosis transmembrane conductance regulator ( CFTR ) is apparently mutually exclusive , particularly in epithelial ; where one protein is expressed the other is not .
	manualset3
167699	6	412812	7	NULL	NULL	0	NULL	epithelial	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The tissue distribution of P-glycoprotein ( Pgp ) and the structurally related cystic fibrosis transmembrane conductance regulator ( CFTR ) is apparently mutually exclusive , particularly in epithelial ; where one protein is expressed the other is not .
	manualset3
167700	1	412813	7	NULL	NULL	0	NULL	Acid secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acid secretion from the completely isolated blood perfused canine stomach .
	manualset3
167701	2	412813	7	NULL	NULL	0	NULL	completely isolated blood 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Acid secretion from the completely isolated blood perfused canine stomach .
	manualset3
167702	3	412813	7	NULL	NULL	0	NULL	canine stomach	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Acid secretion from the completely isolated blood perfused canine stomach .
	manualset3
167703	1	412814	7	NULL	NULL	0	NULL	tissue shear modulus	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The tissue shear modulus , i.e. , its stiffness , can then be estimated from the shear wave local velocity .
	manualset3
167704	2	412814	7	NULL	NULL	0	NULL	stiffness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The tissue shear modulus , i.e. , its stiffness , can then be estimated from the shear wave local velocity .
	manualset3
167705	3	412814	7	NULL	NULL	0	NULL	shear wave local velocity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The tissue shear modulus , i.e. , its stiffness , can then be estimated from the shear wave local velocity .
	manualset3
167706	1	412815	7	NULL	NULL	0	NULL	 titanium dioxide concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The titanium dioxide concentrations were higher for the products of higher SPF values .
	manualset3
167707	2	412815	7	NULL	NULL	0	NULL	products	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The titanium dioxide concentrations were higher for the products of higher SPF values .
	manualset3
167708	3	412815	7	NULL	NULL	0	NULL	higher SPF values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The titanium dioxide concentrations were higher for the products of higher SPF values .
	manualset3
167709	1	412816	7	NULL	NULL	NULL	NULL	tomato transcription factor Pti4	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The tomato transcription factor Pti4 , an ethylene-responsive factor ( ERF ) , interacts physically with the disease resistance protein Pto and binds the GCC box cis element that is present in the promoters of many pathogenesis-related ( PR ) genes .
	manualset3
167710	2	412816	7	NULL	NULL	0	NULL	ethylene-responsive factor ( ERF ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The tomato transcription factor Pti4 , an ethylene-responsive factor ( ERF ) , interacts physically with the disease resistance protein Pto and binds the GCC box cis element that is present in the promoters of many pathogenesis-related ( PR ) genes .
	manualset3
167711	3	412816	7	NULL	NULL	0	NULL	disease resistance protein Pto	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The tomato transcription factor Pti4 , an ethylene-responsive factor ( ERF ) , interacts physically with the disease resistance protein Pto and binds the GCC box cis element that is present in the promoters of many pathogenesis-related ( PR ) genes .
	manualset3
167712	4	412816	7	NULL	NULL	0	NULL	GCC box cis element	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The tomato transcription factor Pti4 , an ethylene-responsive factor ( ERF ) , interacts physically with the disease resistance protein Pto and binds the GCC box cis element that is present in the promoters of many pathogenesis-related ( PR ) genes .
	manualset3
167713	5	412816	7	NULL	NULL	0	NULL	promoters 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The tomato transcription factor Pti4 , an ethylene-responsive factor ( ERF ) , interacts physically with the disease resistance protein Pto and binds the GCC box cis element that is present in the promoters of many pathogenesis-related ( PR ) genes .
	manualset3
167714	6	412816	7	NULL	NULL	0	NULL	pathogenesis-related ( PR ) genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The tomato transcription factor Pti4 , an ethylene-responsive factor ( ERF ) , interacts physically with the disease resistance protein Pto and binds the GCC box cis element that is present in the promoters of many pathogenesis-related ( PR ) genes .
	manualset3
167715	1	412817	7	NULL	NULL	0	NULL	topical application	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The topical application of either drug 5 times daily for 5 days did show a significant difference in surgery mediated disturbance of BAB in each group before and after phacoemulsification .
	manualset3
167716	2	412817	7	NULL	NULL	0	NULL	drug 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The topical application of either drug 5 times daily for 5 days did show a significant difference in surgery mediated disturbance of BAB in each group before and after phacoemulsification .
	manualset3
167717	3	412817	7	NULL	NULL	0	NULL	5 times daily 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The topical application of either drug 5 times daily for 5 days did show a significant difference in surgery mediated disturbance of BAB in each group before and after phacoemulsification .
	manualset3
167718	4	412817	7	NULL	NULL	0	NULL	5 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The topical application of either drug 5 times daily for 5 days did show a significant difference in surgery mediated disturbance of BAB in each group before and after phacoemulsification .
	manualset3
167719	5	412817	7	NULL	NULL	NULL	NULL	surgery mediated disturbance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The topical application of either drug 5 times daily for 5 days did show a significant difference in surgery mediated disturbance of BAB in each group before and after phacoemulsification .
	manualset3
167720	6	412817	7	NULL	NULL	0	NULL	BAB	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The topical application of either drug 5 times daily for 5 days did show a significant difference in surgery mediated disturbance of BAB in each group before and after phacoemulsification .
	manualset3
167721	7	412817	7	NULL	NULL	0	NULL	 group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The topical application of either drug 5 times daily for 5 days did show a significant difference in surgery mediated disturbance of BAB in each group before and after phacoemulsification .
	manualset3
167722	8	412817	7	NULL	NULL	0	NULL	phacoemulsification	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The topical application of either drug 5 times daily for 5 days did show a significant difference in surgery mediated disturbance of BAB in each group before and after phacoemulsification .
	manualset3
167723	1	412818	7	NULL	NULL	0	NULL	topology 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The topology of the tree was ( Fucus serratus ( F. lutarius ( F. vesiculosus ( F. spiralis + F. ceranoides ) ) ) ) .
	manualset3
167724	2	412818	7	NULL	NULL	0	NULL	tree 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The topology of the tree was ( Fucus serratus ( F. lutarius ( F. vesiculosus ( F. spiralis + F. ceranoides ) ) ) ) .
	manualset3
167725	3	412818	7	NULL	NULL	0	NULL	( Fucus serratus ( F. lutarius ( F. vesiculosus ( F. spiralis + F. ceranoides ) ) ) )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The topology of the tree was ( Fucus serratus ( F. lutarius ( F. vesiculosus ( F. spiralis + F. ceranoides ) ) ) ) .
	manualset3
167726	1	412819	7	NULL	NULL	0	NULL	torque	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The torque vs sEMG curves were used to establish the relationship that can be used for detection of the decrease of the force associated with FES-induced muscle fatigue .
	manualset3
167727	2	412819	7	NULL	NULL	0	NULL	sEMG curves	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The torque vs sEMG curves were used to establish the relationship that can be used for detection of the decrease of the force associated with FES-induced muscle fatigue .
	manualset3
167728	3	412819	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The torque vs sEMG curves were used to establish the relationship that can be used for detection of the decrease of the force associated with FES-induced muscle fatigue .
	manualset3
167729	4	412819	7	NULL	NULL	0	NULL	detection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The torque vs sEMG curves were used to establish the relationship that can be used for detection of the decrease of the force associated with FES-induced muscle fatigue .
	manualset3
167730	5	412819	7	NULL	NULL	0	NULL	 decrease of the force	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The torque vs sEMG curves were used to establish the relationship that can be used for detection of the decrease of the force associated with FES-induced muscle fatigue .
	manualset3
167731	6	412819	7	NULL	NULL	0	NULL	FES-induced muscle fatigue	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The torque vs sEMG curves were used to establish the relationship that can be used for detection of the decrease of the force associated with FES-induced muscle fatigue .
	manualset3
167732	1	412820	7	NULL	NULL	NULL	NULL	 total activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The total activity and the isoenzyme fractions of alkaline phosphatase were determined in the serum of 15 patients on intermittent hemodialysis and 32 kidney transplant recipients .
	manualset3
167733	2	412820	7	NULL	NULL	0	NULL	isoenzyme fractions	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The total activity and the isoenzyme fractions of alkaline phosphatase were determined in the serum of 15 patients on intermittent hemodialysis and 32 kidney transplant recipients .
	manualset3
167734	3	412820	7	NULL	NULL	0	NULL	alkaline phosphatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The total activity and the isoenzyme fractions of alkaline phosphatase were determined in the serum of 15 patients on intermittent hemodialysis and 32 kidney transplant recipients .
	manualset3
167735	4	412820	7	NULL	NULL	0	NULL	 serum 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The total activity and the isoenzyme fractions of alkaline phosphatase were determined in the serum of 15 patients on intermittent hemodialysis and 32 kidney transplant recipients .
	manualset3
167736	5	412820	7	NULL	NULL	0	NULL	15 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The total activity and the isoenzyme fractions of alkaline phosphatase were determined in the serum of 15 patients on intermittent hemodialysis and 32 kidney transplant recipients .
	manualset3
167737	6	412820	7	NULL	NULL	0	NULL	intermittent hemodialysis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The total activity and the isoenzyme fractions of alkaline phosphatase were determined in the serum of 15 patients on intermittent hemodialysis and 32 kidney transplant recipients .
	manualset3
167738	7	412820	7	NULL	NULL	0	NULL	32 kidney transplant recipients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The total activity and the isoenzyme fractions of alkaline phosphatase were determined in the serum of 15 patients on intermittent hemodialysis and 32 kidney transplant recipients .
	manualset3
167739	1	412821	7	NULL	NULL	0	NULL	Acidic pectin ( homogalacturonans )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Acidic pectin ( homogalacturonans ) binds calcium and forms chain dimers called egg boxes and even multimers at higher calcium ion concentrations .
	manualset3
167740	2	412821	7	NULL	NULL	0	NULL	calcium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Acidic pectin ( homogalacturonans ) binds calcium and forms chain dimers called egg boxes and even multimers at higher calcium ion concentrations .
	manualset3
167741	3	412821	7	NULL	NULL	0	NULL	chain dimers	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acidic pectin ( homogalacturonans ) binds calcium and forms chain dimers called egg boxes and even multimers at higher calcium ion concentrations .
	manualset3
167742	4	412821	7	NULL	NULL	0	NULL	egg boxes	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Acidic pectin ( homogalacturonans ) binds calcium and forms chain dimers called egg boxes and even multimers at higher calcium ion concentrations .
	manualset3
167743	5	412821	7	NULL	NULL	0	NULL	multimers	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acidic pectin ( homogalacturonans ) binds calcium and forms chain dimers called egg boxes and even multimers at higher calcium ion concentrations .
	manualset3
167744	6	412821	7	NULL	NULL	0	NULL	calcium ion concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Acidic pectin ( homogalacturonans ) binds calcium and forms chain dimers called egg boxes and even multimers at higher calcium ion concentrations .
	manualset3
167745	1	412822	7	NULL	NULL	0	NULL	total amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The total amount of ascorbate did not increase , however , implying modified ascorbate turnover .
	manualset3
167746	2	412822	7	NULL	NULL	0	NULL	ascorbate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The total amount of ascorbate did not increase , however , implying modified ascorbate turnover .
	manualset3
167747	3	412822	7	NULL	NULL	0	NULL	ascorbate turnover	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The total amount of ascorbate did not increase , however , implying modified ascorbate turnover .
	manualset3
167748	1	412823	7	NULL	NULL	0	NULL	total concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The total concentration of hydrocarbons is a simple and convenient measure of exposure , which also seems to be a predictor of chronic symptoms .
	manualset3
167749	2	412823	7	NULL	NULL	0	NULL	hydrocarbons	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The total concentration of hydrocarbons is a simple and convenient measure of exposure , which also seems to be a predictor of chronic symptoms .
	manualset3
167750	3	412823	7	NULL	NULL	0	NULL	measure of exposure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The total concentration of hydrocarbons is a simple and convenient measure of exposure , which also seems to be a predictor of chronic symptoms .
	manualset3
167751	4	412823	7	NULL	NULL	0	NULL	predictor 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The total concentration of hydrocarbons is a simple and convenient measure of exposure , which also seems to be a predictor of chronic symptoms .
	manualset3
167752	5	412823	7	NULL	NULL	0	NULL	chronic symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The total concentration of hydrocarbons is a simple and convenient measure of exposure , which also seems to be a predictor of chronic symptoms .
	manualset3
167753	1	412824	7	NULL	NULL	0	NULL	total concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The total concentrations of delta 1-THC-7-oic acid in urine were compared to the concentrations of `` cross-reacting cannabinoids '' , within the linear range of 20-75 ng/mL , obtained in the semiquantitative EMIT d.a.u. cannabinoid assay .
	manualset3
167754	2	412824	7	NULL	NULL	0	NULL	delta 1-THC-7-oic acid 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The total concentrations of delta 1-THC-7-oic acid in urine were compared to the concentrations of `` cross-reacting cannabinoids '' , within the linear range of 20-75 ng/mL , obtained in the semiquantitative EMIT d.a.u. cannabinoid assay .
	manualset3
167755	3	412824	7	NULL	NULL	0	NULL	urine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The total concentrations of delta 1-THC-7-oic acid in urine were compared to the concentrations of `` cross-reacting cannabinoids '' , within the linear range of 20-75 ng/mL , obtained in the semiquantitative EMIT d.a.u. cannabinoid assay .
	manualset3
167756	4	412824	7	NULL	NULL	0	NULL	concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The total concentrations of delta 1-THC-7-oic acid in urine were compared to the concentrations of `` cross-reacting cannabinoids '' , within the linear range of 20-75 ng/mL , obtained in the semiquantitative EMIT d.a.u. cannabinoid assay .
	manualset3
167757	5	412824	7	NULL	NULL	0	NULL	cross-reacting cannabinoids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The total concentrations of delta 1-THC-7-oic acid in urine were compared to the concentrations of `` cross-reacting cannabinoids '' , within the linear range of 20-75 ng/mL , obtained in the semiquantitative EMIT d.a.u. cannabinoid assay .
	manualset3
167758	6	412824	7	NULL	NULL	0	NULL	linear range	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The total concentrations of delta 1-THC-7-oic acid in urine were compared to the concentrations of `` cross-reacting cannabinoids '' , within the linear range of 20-75 ng/mL , obtained in the semiquantitative EMIT d.a.u. cannabinoid assay .
	manualset3
167759	7	412824	7	NULL	NULL	0	NULL	20-75 ng/mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The total concentrations of delta 1-THC-7-oic acid in urine were compared to the concentrations of `` cross-reacting cannabinoids '' , within the linear range of 20-75 ng/mL , obtained in the semiquantitative EMIT d.a.u. cannabinoid assay .
	manualset3
167760	8	412824	7	NULL	NULL	0	NULL	semiquantitative EMIT d.a.u. cannabinoid assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The total concentrations of delta 1-THC-7-oic acid in urine were compared to the concentrations of `` cross-reacting cannabinoids '' , within the linear range of 20-75 ng/mL , obtained in the semiquantitative EMIT d.a.u. cannabinoid assay .
	manualset3
167761	1	412825	7	NULL	NULL	0	NULL	 total dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The total dose ranged from 5.4 to 74 Gy ( mean , 41.4 Gy ) .
	manualset3
167762	2	412825	7	NULL	NULL	0	NULL	5.4 to 74 Gy	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The total dose ranged from 5.4 to 74 Gy ( mean , 41.4 Gy ) .
	manualset3
167763	3	412825	7	NULL	NULL	0	NULL	 mean 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The total dose ranged from 5.4 to 74 Gy ( mean , 41.4 Gy ) .
	manualset3
167764	4	412825	7	NULL	NULL	0	NULL	41.4 Gy	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The total dose ranged from 5.4 to 74 Gy ( mean , 41.4 Gy ) .
	manualset3
167765	1	412826	7	NULL	NULL	0	NULL	total hexokinase activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The total hexokinase activity increases , whereas that of total glycogen phosphorylase decreases .
	manualset3
167766	2	412826	7	NULL	NULL	0	NULL	 total glycogen phosphorylase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The total hexokinase activity increases , whereas that of total glycogen phosphorylase decreases .
	manualset3
167767	1	412827	7	NULL	NULL	0	NULL	 total number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The total number of CIK cells used ranged from 610 ( 6 ) to 1.510 ( 10 ) .
	manualset3
167768	2	412827	7	NULL	NULL	0	NULL	CIK cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The total number of CIK cells used ranged from 610 ( 6 ) to 1.510 ( 10 ) .
	manualset3
167769	3	412827	7	NULL	NULL	0	NULL	610 ( 6 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The total number of CIK cells used ranged from 610 ( 6 ) to 1.510 ( 10 ) .
	manualset3
167770	4	412827	7	NULL	NULL	0	NULL	1.510 ( 10 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The total number of CIK cells used ranged from 610 ( 6 ) to 1.510 ( 10 ) .
	manualset3
167771	1	412828	7	NULL	NULL	0	NULL	total number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The total number of malaria patients in Vietnam has gradually decreased over the last decade .
	manualset3
167772	2	412828	7	NULL	NULL	0	NULL	malaria patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The total number of malaria patients in Vietnam has gradually decreased over the last decade .
	manualset3
167773	3	412828	7	NULL	NULL	0	NULL	Vietnam	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The total number of malaria patients in Vietnam has gradually decreased over the last decade .
	manualset3
167774	4	412828	7	NULL	NULL	0	NULL	decade	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The total number of malaria patients in Vietnam has gradually decreased over the last decade .
	manualset3
167775	1	412829	7	NULL	NULL	0	NULL	Colon cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Colon cancer : a new French medical affair ? ) .
	manualset3
167776	2	412829	7	NULL	NULL	0	NULL	a new French medical affair ?	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Colon cancer : a new French medical affair ? ) .
	manualset3
167777	1	412830	7	NULL	NULL	0	NULL	legitimate forces basic changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Acknowledging these interests as legitimate forces basic changes in ethical theory and the moral practice of medicine .
	manualset3
167778	2	412830	7	NULL	NULL	0	NULL	ethical theory	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Acknowledging these interests as legitimate forces basic changes in ethical theory and the moral practice of medicine .
	manualset3
167779	3	412830	7	NULL	NULL	0	NULL	moral practice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Acknowledging these interests as legitimate forces basic changes in ethical theory and the moral practice of medicine .
	manualset3
167780	4	412830	7	NULL	NULL	0	NULL	medicine	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Acknowledging these interests as legitimate forces basic changes in ethical theory and the moral practice of medicine .
	manualset3
173655	5	412830	7	NULL	NULL	0	NULL	interests	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acknowledging these interests as legitimate forces basic changes in ethical theory and the moral practice of medicine .
	manualset3
167791	1	412831	7	NULL	NULL	0	NULL	total polyunsaturated fatty acid content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The total polyunsaturated fatty acid content and the n-6 to n-3 polyunsaturated fatty acid ratio of the diet were maintained at 35 g/100 g total fatty acids and 7 , respectively .
	manualset3
167792	2	412831	7	NULL	NULL	0	NULL	n-6 to n-3 polyunsaturated fatty acid ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The total polyunsaturated fatty acid content and the n-6 to n-3 polyunsaturated fatty acid ratio of the diet were maintained at 35 g/100 g total fatty acids and 7 , respectively .
	manualset3
167793	3	412831	7	NULL	NULL	0	NULL	diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The total polyunsaturated fatty acid content and the n-6 to n-3 polyunsaturated fatty acid ratio of the diet were maintained at 35 g/100 g total fatty acids and 7 , respectively .
	manualset3
167794	4	412831	7	NULL	NULL	0	NULL	35 g/100 g	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The total polyunsaturated fatty acid content and the n-6 to n-3 polyunsaturated fatty acid ratio of the diet were maintained at 35 g/100 g total fatty acids and 7 , respectively .
	manualset3
167795	5	412831	7	NULL	NULL	0	NULL	total fatty acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The total polyunsaturated fatty acid content and the n-6 to n-3 polyunsaturated fatty acid ratio of the diet were maintained at 35 g/100 g total fatty acids and 7 , respectively .
	manualset3
167796	6	412831	7	NULL	NULL	0	NULL	7	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The total polyunsaturated fatty acid content and the n-6 to n-3 polyunsaturated fatty acid ratio of the diet were maintained at 35 g/100 g total fatty acids and 7 , respectively .
	manualset3
167797	1	412832	7	NULL	NULL	0	NULL	 total protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The total protein and total activity , on the other hand , decrease more and more rapidly up to about 70 degrees C. but as the temperature is raised above this there is less rapid change in the total protein or total activity and at 92 degrees C. the solutions are much more stable than at 42 degrees C. 4 .
	manualset3
167798	2	412832	7	NULL	NULL	0	NULL	 total activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The total protein and total activity , on the other hand , decrease more and more rapidly up to about 70 degrees C. but as the temperature is raised above this there is less rapid change in the total protein or total activity and at 92 degrees C. the solutions are much more stable than at 42 degrees C. 4 .
	manualset3
167799	3	412832	7	NULL	NULL	0	NULL	70 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The total protein and total activity , on the other hand , decrease more and more rapidly up to about 70 degrees C. but as the temperature is raised above this there is less rapid change in the total protein or total activity and at 92 degrees C. the solutions are much more stable than at 42 degrees C. 4 .
	manualset3
167800	4	412832	7	NULL	NULL	NULL	NULL	 temperature	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The total protein and total activity , on the other hand , decrease more and more rapidly up to about 70 degrees C. but as the temperature is raised above this there is less rapid change in the total protein or total activity and at 92 degrees C. the solutions are much more stable than at 42 degrees C. 4 .
	manualset3
167801	5	412832	7	NULL	NULL	0	NULL	rapid change	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The total protein and total activity , on the other hand , decrease more and more rapidly up to about 70 degrees C. but as the temperature is raised above this there is less rapid change in the total protein or total activity and at 92 degrees C. the solutions are much more stable than at 42 degrees C. 4 .
	manualset3
167802	6	412832	7	NULL	NULL	0	NULL	total protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The total protein and total activity , on the other hand , decrease more and more rapidly up to about 70 degrees C. but as the temperature is raised above this there is less rapid change in the total protein or total activity and at 92 degrees C. the solutions are much more stable than at 42 degrees C. 4 .
	manualset3
167803	7	412832	7	NULL	NULL	0	NULL	total activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The total protein and total activity , on the other hand , decrease more and more rapidly up to about 70 degrees C. but as the temperature is raised above this there is less rapid change in the total protein or total activity and at 92 degrees C. the solutions are much more stable than at 42 degrees C. 4 .
	manualset3
167804	8	412832	7	NULL	NULL	0	NULL	92 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The total protein and total activity , on the other hand , decrease more and more rapidly up to about 70 degrees C. but as the temperature is raised above this there is less rapid change in the total protein or total activity and at 92 degrees C. the solutions are much more stable than at 42 degrees C. 4 .
	manualset3
167805	9	412832	7	NULL	NULL	0	NULL	solutions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The total protein and total activity , on the other hand , decrease more and more rapidly up to about 70 degrees C. but as the temperature is raised above this there is less rapid change in the total protein or total activity and at 92 degrees C. the solutions are much more stable than at 42 degrees C. 4 .
	manualset3
167806	10	412832	7	NULL	NULL	0	NULL	42 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The total protein and total activity , on the other hand , decrease more and more rapidly up to about 70 degrees C. but as the temperature is raised above this there is less rapid change in the total protein or total activity and at 92 degrees C. the solutions are much more stable than at 42 degrees C. 4 .
	manualset3
167807	1	412833	7	NULL	NULL	0	NULL	total protein determination method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The total protein determination method was only sensitive enough to detect the antiproliferative influence of tamoxifen at concentrations above 10 ( -6 ) M. In conclusion , the ( 3H ) - thymidine incorporation method was found to be effective and much less time consuming than the hemocytometric trypan blue exclusion method for evaluating the antiproliferative effects of antiestrogens in cultured MCF-7 cells .
	manualset3
167808	2	412833	7	NULL	NULL	0	NULL	antiproliferative influence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The total protein determination method was only sensitive enough to detect the antiproliferative influence of tamoxifen at concentrations above 10 ( -6 ) M. In conclusion , the ( 3H ) - thymidine incorporation method was found to be effective and much less time consuming than the hemocytometric trypan blue exclusion method for evaluating the antiproliferative effects of antiestrogens in cultured MCF-7 cells .
	manualset3
167809	3	412833	7	NULL	NULL	0	NULL	tamoxifen	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The total protein determination method was only sensitive enough to detect the antiproliferative influence of tamoxifen at concentrations above 10 ( -6 ) M. In conclusion , the ( 3H ) - thymidine incorporation method was found to be effective and much less time consuming than the hemocytometric trypan blue exclusion method for evaluating the antiproliferative effects of antiestrogens in cultured MCF-7 cells .
	manualset3
167810	4	412833	7	NULL	NULL	0	NULL	concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The total protein determination method was only sensitive enough to detect the antiproliferative influence of tamoxifen at concentrations above 10 ( -6 ) M. In conclusion , the ( 3H ) - thymidine incorporation method was found to be effective and much less time consuming than the hemocytometric trypan blue exclusion method for evaluating the antiproliferative effects of antiestrogens in cultured MCF-7 cells .
	manualset3
167811	5	412833	7	NULL	NULL	0	NULL	 10 ( -6 ) M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The total protein determination method was only sensitive enough to detect the antiproliferative influence of tamoxifen at concentrations above 10 ( -6 ) M. In conclusion , the ( 3H ) - thymidine incorporation method was found to be effective and much less time consuming than the hemocytometric trypan blue exclusion method for evaluating the antiproliferative effects of antiestrogens in cultured MCF-7 cells .
	manualset3
167812	6	412833	7	NULL	NULL	0	NULL	conclusion	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The total protein determination method was only sensitive enough to detect the antiproliferative influence of tamoxifen at concentrations above 10 ( -6 ) M. In conclusion , the ( 3H ) - thymidine incorporation method was found to be effective and much less time consuming than the hemocytometric trypan blue exclusion method for evaluating the antiproliferative effects of antiestrogens in cultured MCF-7 cells .
	manualset3
167813	7	412833	7	NULL	NULL	0	NULL	( 3H ) - thymidine incorporation method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The total protein determination method was only sensitive enough to detect the antiproliferative influence of tamoxifen at concentrations above 10 ( -6 ) M. In conclusion , the ( 3H ) - thymidine incorporation method was found to be effective and much less time consuming than the hemocytometric trypan blue exclusion method for evaluating the antiproliferative effects of antiestrogens in cultured MCF-7 cells .
	manualset3
167814	8	412833	7	NULL	NULL	0	NULL	hemocytometric trypan blue exclusion method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The total protein determination method was only sensitive enough to detect the antiproliferative influence of tamoxifen at concentrations above 10 ( -6 ) M. In conclusion , the ( 3H ) - thymidine incorporation method was found to be effective and much less time consuming than the hemocytometric trypan blue exclusion method for evaluating the antiproliferative effects of antiestrogens in cultured MCF-7 cells .
	manualset3
167815	9	412833	7	NULL	NULL	0	NULL	evaluating	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The total protein determination method was only sensitive enough to detect the antiproliferative influence of tamoxifen at concentrations above 10 ( -6 ) M. In conclusion , the ( 3H ) - thymidine incorporation method was found to be effective and much less time consuming than the hemocytometric trypan blue exclusion method for evaluating the antiproliferative effects of antiestrogens in cultured MCF-7 cells .
	manualset3
167816	10	412833	7	NULL	NULL	0	NULL	antiproliferative effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The total protein determination method was only sensitive enough to detect the antiproliferative influence of tamoxifen at concentrations above 10 ( -6 ) M. In conclusion , the ( 3H ) - thymidine incorporation method was found to be effective and much less time consuming than the hemocytometric trypan blue exclusion method for evaluating the antiproliferative effects of antiestrogens in cultured MCF-7 cells .
	manualset3
167817	11	412833	7	NULL	NULL	0	NULL	antiestrogens	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The total protein determination method was only sensitive enough to detect the antiproliferative influence of tamoxifen at concentrations above 10 ( -6 ) M. In conclusion , the ( 3H ) - thymidine incorporation method was found to be effective and much less time consuming than the hemocytometric trypan blue exclusion method for evaluating the antiproliferative effects of antiestrogens in cultured MCF-7 cells .
	manualset3
167818	12	412833	7	NULL	NULL	0	NULL	cultured MCF-7 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The total protein determination method was only sensitive enough to detect the antiproliferative influence of tamoxifen at concentrations above 10 ( -6 ) M. In conclusion , the ( 3H ) - thymidine incorporation method was found to be effective and much less time consuming than the hemocytometric trypan blue exclusion method for evaluating the antiproliferative effects of antiestrogens in cultured MCF-7 cells .
	manualset3
167819	1	412834	7	NULL	NULL	0	NULL	 total time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The total time of test solving was correlated with Dialysis Malnutrition Score ( DMS ) in tests of simple visual discrimination of signal location ( r = 0.215 , P = 0.042 ) , simple convergent visual orientation ( r = 0.262 , P = 0.020 ) , and convergent thinking ( r = 0.244 , P = 0.034 ) .
	manualset3
167820	2	412834	7	NULL	NULL	NULL	NULL	test	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The total time of test solving was correlated with Dialysis Malnutrition Score ( DMS ) in tests of simple visual discrimination of signal location ( r = 0.215 , P = 0.042 ) , simple convergent visual orientation ( r = 0.262 , P = 0.020 ) , and convergent thinking ( r = 0.244 , P = 0.034 ) .
	manualset3
167821	3	412834	7	NULL	NULL	NULL	NULL	Dialysis Malnutrition Score ( DMS )	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The total time of test solving was correlated with Dialysis Malnutrition Score ( DMS ) in tests of simple visual discrimination of signal location ( r = 0.215 , P = 0.042 ) , simple convergent visual orientation ( r = 0.262 , P = 0.020 ) , and convergent thinking ( r = 0.244 , P = 0.034 ) .
	manualset3
167822	4	412834	7	NULL	NULL	NULL	NULL	tests	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The total time of test solving was correlated with Dialysis Malnutrition Score ( DMS ) in tests of simple visual discrimination of signal location ( r = 0.215 , P = 0.042 ) , simple convergent visual orientation ( r = 0.262 , P = 0.020 ) , and convergent thinking ( r = 0.244 , P = 0.034 ) .
	manualset3
167823	5	412834	7	NULL	NULL	0	NULL	simple visual discrimination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The total time of test solving was correlated with Dialysis Malnutrition Score ( DMS ) in tests of simple visual discrimination of signal location ( r = 0.215 , P = 0.042 ) , simple convergent visual orientation ( r = 0.262 , P = 0.020 ) , and convergent thinking ( r = 0.244 , P = 0.034 ) .
	manualset3
167824	6	412834	7	NULL	NULL	0	NULL	signal location	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The total time of test solving was correlated with Dialysis Malnutrition Score ( DMS ) in tests of simple visual discrimination of signal location ( r = 0.215 , P = 0.042 ) , simple convergent visual orientation ( r = 0.262 , P = 0.020 ) , and convergent thinking ( r = 0.244 , P = 0.034 ) .
	manualset3
167825	7	412834	7	NULL	NULL	0	NULL	 r = 0.215 , P = 0.042	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The total time of test solving was correlated with Dialysis Malnutrition Score ( DMS ) in tests of simple visual discrimination of signal location ( r = 0.215 , P = 0.042 ) , simple convergent visual orientation ( r = 0.262 , P = 0.020 ) , and convergent thinking ( r = 0.244 , P = 0.034 ) .
	manualset3
167826	8	412834	7	NULL	NULL	NULL	NULL	simple convergent visual orientation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The total time of test solving was correlated with Dialysis Malnutrition Score ( DMS ) in tests of simple visual discrimination of signal location ( r = 0.215 , P = 0.042 ) , simple convergent visual orientation ( r = 0.262 , P = 0.020 ) , and convergent thinking ( r = 0.244 , P = 0.034 ) .
	manualset3
167827	9	412834	7	NULL	NULL	0	NULL	 r = 0.262 , P = 0.020	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The total time of test solving was correlated with Dialysis Malnutrition Score ( DMS ) in tests of simple visual discrimination of signal location ( r = 0.215 , P = 0.042 ) , simple convergent visual orientation ( r = 0.262 , P = 0.020 ) , and convergent thinking ( r = 0.244 , P = 0.034 ) .
	manualset3
167828	10	412834	7	NULL	NULL	0	NULL	convergent thinking	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The total time of test solving was correlated with Dialysis Malnutrition Score ( DMS ) in tests of simple visual discrimination of signal location ( r = 0.215 , P = 0.042 ) , simple convergent visual orientation ( r = 0.262 , P = 0.020 ) , and convergent thinking ( r = 0.244 , P = 0.034 ) .
	manualset3
167829	11	412834	7	NULL	NULL	0	NULL	r = 0.244 , P = 0.034	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The total time of test solving was correlated with Dialysis Malnutrition Score ( DMS ) in tests of simple visual discrimination of signal location ( r = 0.215 , P = 0.042 ) , simple convergent visual orientation ( r = 0.262 , P = 0.020 ) , and convergent thinking ( r = 0.244 , P = 0.034 ) .
	manualset3
167830	1	412835	7	NULL	NULL	0	NULL	toxicity profile	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The toxicity profile is acceptable without serious symptoms .
	manualset3
167831	2	412835	7	NULL	NULL	0	NULL	serious symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The toxicity profile is acceptable without serious symptoms .
	manualset3
167832	1	412836	7	NULL	NULL	0	NULL	 toxicology	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The toxicology of OPs was interpreted until recently almost solely on the basis of AChE inhibition .
	manualset3
167833	2	412836	7	NULL	NULL	0	NULL	OPs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The toxicology of OPs was interpreted until recently almost solely on the basis of AChE inhibition .
	manualset3
167834	3	412836	7	NULL	NULL	0	NULL	basis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The toxicology of OPs was interpreted until recently almost solely on the basis of AChE inhibition .
	manualset3
167835	4	412836	7	NULL	NULL	0	NULL	AChE inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The toxicology of OPs was interpreted until recently almost solely on the basis of AChE inhibition .
	manualset3
167836	1	412837	7	NULL	NULL	0	NULL	Aclacinomycin A	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Aclacinomycin A showed a marked antitumor effect on AH 41 C in the iv-iv system , and AH 44 in the iv-ip and iv-po systems .
	manualset3
167837	2	412837	7	NULL	NULL	0	NULL	antitumor effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Aclacinomycin A showed a marked antitumor effect on AH 41 C in the iv-iv system , and AH 44 in the iv-ip and iv-po systems .
	manualset3
167838	3	412837	7	NULL	NULL	0	NULL	AH 41 C	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Aclacinomycin A showed a marked antitumor effect on AH 41 C in the iv-iv system , and AH 44 in the iv-ip and iv-po systems .
	manualset3
167839	4	412837	7	NULL	NULL	0	NULL	 iv-iv system	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Aclacinomycin A showed a marked antitumor effect on AH 41 C in the iv-iv system , and AH 44 in the iv-ip and iv-po systems .
	manualset3
167840	5	412837	7	NULL	NULL	0	NULL	AH 44	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Aclacinomycin A showed a marked antitumor effect on AH 41 C in the iv-iv system , and AH 44 in the iv-ip and iv-po systems .
	manualset3
167841	6	412837	7	NULL	NULL	0	NULL	 iv-ip system	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Aclacinomycin A showed a marked antitumor effect on AH 41 C in the iv-iv system , and AH 44 in the iv-ip and iv-po systems .
	manualset3
167842	7	412837	7	NULL	NULL	0	NULL	iv-po systems	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Aclacinomycin A showed a marked antitumor effect on AH 41 C in the iv-iv system , and AH 44 in the iv-ip and iv-po systems .
	manualset3
167843	1	412838	7	NULL	NULL	0	NULL	 tracer	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The tracer was stable for 24 hours in human and mouse serum at 37C .
	manualset3
167844	2	412838	7	NULL	NULL	0	NULL	24 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The tracer was stable for 24 hours in human and mouse serum at 37C .
	manualset3
167845	3	412838	7	NULL	NULL	NULL	NULL	human serum	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The tracer was stable for 24 hours in human and mouse serum at 37C .
	manualset3
167846	4	412838	7	NULL	NULL	0	NULL	mouse serum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The tracer was stable for 24 hours in human and mouse serum at 37C .
	manualset3
167847	5	412838	7	NULL	NULL	0	NULL	37C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The tracer was stable for 24 hours in human and mouse serum at 37C .
	manualset3
167848	1	412839	7	NULL	NULL	0	NULL	training	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The training at the Institute of Development Studies at the University of Sussex focused on rules , practices , access to resources , and formal and informal inclusions and exclusions .
	manualset3
167849	2	412839	7	NULL	NULL	0	NULL	Institute of Development Studies	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The training at the Institute of Development Studies at the University of Sussex focused on rules , practices , access to resources , and formal and informal inclusions and exclusions .
	manualset3
167850	3	412839	7	NULL	NULL	0	NULL	University of Sussex	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The training at the Institute of Development Studies at the University of Sussex focused on rules , practices , access to resources , and formal and informal inclusions and exclusions .
	manualset3
167851	4	412839	7	NULL	NULL	0	NULL	rules	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The training at the Institute of Development Studies at the University of Sussex focused on rules , practices , access to resources , and formal and informal inclusions and exclusions .
	manualset3
167852	5	412839	7	NULL	NULL	0	NULL	practices	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The training at the Institute of Development Studies at the University of Sussex focused on rules , practices , access to resources , and formal and informal inclusions and exclusions .
	manualset3
167853	6	412839	7	NULL	NULL	0	NULL	access to resources	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The training at the Institute of Development Studies at the University of Sussex focused on rules , practices , access to resources , and formal and informal inclusions and exclusions .
	manualset3
167854	7	412839	7	NULL	NULL	NULL	NULL	formal inclusion	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The training at the Institute of Development Studies at the University of Sussex focused on rules , practices , access to resources , and formal and informal inclusions and exclusions .
	manualset3
167855	8	412839	7	NULL	NULL	0	NULL	informal inclusions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The training at the Institute of Development Studies at the University of Sussex focused on rules , practices , access to resources , and formal and informal inclusions and exclusions .
	manualset3
167856	9	412839	7	NULL	NULL	0	NULL	formal exclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The training at the Institute of Development Studies at the University of Sussex focused on rules , practices , access to resources , and formal and informal inclusions and exclusions .
	manualset3
167857	10	412839	7	NULL	NULL	0	NULL	 informal exclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The training at the Institute of Development Studies at the University of Sussex focused on rules , practices , access to resources , and formal and informal inclusions and exclusions .
	manualset3
167858	1	412840	7	NULL	NULL	0	NULL	trajectory	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The trajectory of the disassembly process differs for the monomeric and dimerizing set of proteins .
	manualset3
167859	2	412840	7	NULL	NULL	0	NULL	disassembly process	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The trajectory of the disassembly process differs for the monomeric and dimerizing set of proteins .
	manualset3
167860	3	412840	7	NULL	NULL	0	NULL	monomeric set	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The trajectory of the disassembly process differs for the monomeric and dimerizing set of proteins .
	manualset3
167861	4	412840	7	NULL	NULL	0	NULL	dimerizing set	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The trajectory of the disassembly process differs for the monomeric and dimerizing set of proteins .
	manualset3
167862	5	412840	7	NULL	NULL	0	NULL	proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The trajectory of the disassembly process differs for the monomeric and dimerizing set of proteins .
	manualset3
167863	1	412841	7	NULL	NULL	0	NULL	transcription elongation factor S-II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The transcription elongation factor S-II , also designated TFIIS , stimulates the nascent transcript cleavage activity intrinsic to RNA polymerase II .
	manualset3
167864	2	412841	7	NULL	NULL	0	NULL	TFIIS	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The transcription elongation factor S-II , also designated TFIIS , stimulates the nascent transcript cleavage activity intrinsic to RNA polymerase II .
	manualset3
167865	3	412841	7	NULL	NULL	0	NULL	nascent transcript cleavage activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The transcription elongation factor S-II , also designated TFIIS , stimulates the nascent transcript cleavage activity intrinsic to RNA polymerase II .
	manualset3
167866	4	412841	7	NULL	NULL	0	NULL	RNA polymerase II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The transcription elongation factor S-II , also designated TFIIS , stimulates the nascent transcript cleavage activity intrinsic to RNA polymerase II .
	manualset3
167867	1	412842	7	NULL	NULL	0	NULL	 transcription factor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The transcription factor , NFkB , plays a pivotal role in the coordinated transactivation of cytokine and adhesion molecule genes involved in atherosclerosis and lesion formation after vascular injury .
	manualset3
167868	2	412842	7	NULL	NULL	0	NULL	NFkB	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The transcription factor , NFkB , plays a pivotal role in the coordinated transactivation of cytokine and adhesion molecule genes involved in atherosclerosis and lesion formation after vascular injury .
	manualset3
167869	3	412842	7	NULL	NULL	0	NULL	 role 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The transcription factor , NFkB , plays a pivotal role in the coordinated transactivation of cytokine and adhesion molecule genes involved in atherosclerosis and lesion formation after vascular injury .
	manualset3
167870	4	412842	7	NULL	NULL	0	NULL	coordinated transactivation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The transcription factor , NFkB , plays a pivotal role in the coordinated transactivation of cytokine and adhesion molecule genes involved in atherosclerosis and lesion formation after vascular injury .
	manualset3
167871	5	412842	7	NULL	NULL	0	NULL	cytokine	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The transcription factor , NFkB , plays a pivotal role in the coordinated transactivation of cytokine and adhesion molecule genes involved in atherosclerosis and lesion formation after vascular injury .
	manualset3
167872	6	412842	7	NULL	NULL	0	NULL	 adhesion molecule genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The transcription factor , NFkB , plays a pivotal role in the coordinated transactivation of cytokine and adhesion molecule genes involved in atherosclerosis and lesion formation after vascular injury .
	manualset3
167873	7	412842	7	NULL	NULL	0	NULL	atherosclerosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The transcription factor , NFkB , plays a pivotal role in the coordinated transactivation of cytokine and adhesion molecule genes involved in atherosclerosis and lesion formation after vascular injury .
	manualset3
167874	8	412842	7	NULL	NULL	0	NULL	lesion formation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The transcription factor , NFkB , plays a pivotal role in the coordinated transactivation of cytokine and adhesion molecule genes involved in atherosclerosis and lesion formation after vascular injury .
	manualset3
167875	9	412842	7	NULL	NULL	0	NULL	vascular injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The transcription factor , NFkB , plays a pivotal role in the coordinated transactivation of cytokine and adhesion molecule genes involved in atherosclerosis and lesion formation after vascular injury .
	manualset3
167876	1	412843	7	NULL	NULL	0	NULL	transcription factor Ets-1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The transcription factor Ets-1 regulates the expression of several genes involved in extracellular matrix remodeling that may account for its association with lymph node and distant organ metastasis .
	manualset3
167877	2	412843	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The transcription factor Ets-1 regulates the expression of several genes involved in extracellular matrix remodeling that may account for its association with lymph node and distant organ metastasis .
	manualset3
167878	3	412843	7	NULL	NULL	0	NULL	genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The transcription factor Ets-1 regulates the expression of several genes involved in extracellular matrix remodeling that may account for its association with lymph node and distant organ metastasis .
	manualset3
167879	4	412843	7	NULL	NULL	0	NULL	extracellular matrix remodeling	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The transcription factor Ets-1 regulates the expression of several genes involved in extracellular matrix remodeling that may account for its association with lymph node and distant organ metastasis .
	manualset3
167880	5	412843	7	NULL	NULL	0	NULL	association	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The transcription factor Ets-1 regulates the expression of several genes involved in extracellular matrix remodeling that may account for its association with lymph node and distant organ metastasis .
	manualset3
167881	6	412843	7	NULL	NULL	0	NULL	lymph node	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The transcription factor Ets-1 regulates the expression of several genes involved in extracellular matrix remodeling that may account for its association with lymph node and distant organ metastasis .
	manualset3
167882	7	412843	7	NULL	NULL	0	NULL	 distant organ metastasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The transcription factor Ets-1 regulates the expression of several genes involved in extracellular matrix remodeling that may account for its association with lymph node and distant organ metastasis .
	manualset3
167883	1	412844	7	NULL	NULL	0	NULL	 transcription factor Pet-1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The transcription factor Pet-1 is an early developmental indicator of neurons that are destined for a 5-HTergic fate .
	manualset3
167884	2	412844	7	NULL	NULL	0	NULL	early developmental indicator	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The transcription factor Pet-1 is an early developmental indicator of neurons that are destined for a 5-HTergic fate .
	manualset3
167885	3	412844	7	NULL	NULL	0	NULL	neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The transcription factor Pet-1 is an early developmental indicator of neurons that are destined for a 5-HTergic fate .
	manualset3
167886	4	412844	7	NULL	NULL	0	NULL	5-HTergic fate	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The transcription factor Pet-1 is an early developmental indicator of neurons that are destined for a 5-HTergic fate .
	manualset3
167887	1	412845	7	NULL	NULL	0	NULL	transcription start site	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The transcription start site of the waxy gene in O. sativa subsp .
	manualset3
167888	2	412845	7	NULL	NULL	0	NULL	waxy gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The transcription start site of the waxy gene in O. sativa subsp .
	manualset3
167889	3	412845	7	NULL	NULL	0	NULL	O. sativa subsp	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The transcription start site of the waxy gene in O. sativa subsp .
	manualset3
167890	1	412846	7	NULL	NULL	0	NULL	Aconitase enzyme activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Aconitase enzyme activity was decreased to approximately 50 % of that observed in isograft controls by POD4 .
	manualset3
167891	2	412846	7	NULL	NULL	0	NULL	50 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Aconitase enzyme activity was decreased to approximately 50 % of that observed in isograft controls by POD4 .
	manualset3
167892	3	412846	7	NULL	NULL	NULL	NULL	isograft controls	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Aconitase enzyme activity was decreased to approximately 50 % of that observed in isograft controls by POD4 .
	manualset3
167893	4	412846	7	NULL	NULL	0	NULL	 POD4	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Aconitase enzyme activity was decreased to approximately 50 % of that observed in isograft controls by POD4 .
	manualset3
167894	1	412847	7	NULL	NULL	0	NULL	 transducing activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The transducing activity of the pseudotyped viruses was not inhibited by neuraminidase treatment of the permissive recipient cells , in contrast to that of virions packaged using LuIII capsid proteins .
	manualset3
167895	2	412847	7	NULL	NULL	0	NULL	pseudotyped viruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The transducing activity of the pseudotyped viruses was not inhibited by neuraminidase treatment of the permissive recipient cells , in contrast to that of virions packaged using LuIII capsid proteins .
	manualset3
167896	3	412847	7	NULL	NULL	NULL	NULL	neuraminidase treatment	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The transducing activity of the pseudotyped viruses was not inhibited by neuraminidase treatment of the permissive recipient cells , in contrast to that of virions packaged using LuIII capsid proteins .
	manualset3
167897	4	412847	7	NULL	NULL	0	NULL	permissive recipient cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The transducing activity of the pseudotyped viruses was not inhibited by neuraminidase treatment of the permissive recipient cells , in contrast to that of virions packaged using LuIII capsid proteins .
	manualset3
167898	5	412847	7	NULL	NULL	0	NULL	virions	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The transducing activity of the pseudotyped viruses was not inhibited by neuraminidase treatment of the permissive recipient cells , in contrast to that of virions packaged using LuIII capsid proteins .
	manualset3
167899	6	412847	7	NULL	NULL	0	NULL	LuIII capsid proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The transducing activity of the pseudotyped viruses was not inhibited by neuraminidase treatment of the permissive recipient cells , in contrast to that of virions packaged using LuIII capsid proteins .
	manualset3
167900	1	412848	7	NULL	NULL	NULL	NULL	 transduction pathways	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The transduction pathways coupling muscarinic receptors to induction of fos and jun genes were investigated in neuroblastoma SH-SY5Y cells .
	manualset3
167901	2	412848	7	NULL	NULL	NULL	NULL	muscarinic receptors	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The transduction pathways coupling muscarinic receptors to induction of fos and jun genes were investigated in neuroblastoma SH-SY5Y cells .
	manualset3
167902	3	412848	7	NULL	NULL	NULL	NULL	fos genes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The transduction pathways coupling muscarinic receptors to induction of fos and jun genes were investigated in neuroblastoma SH-SY5Y cells .
	manualset3
167903	4	412848	7	NULL	NULL	NULL	NULL	jun genes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The transduction pathways coupling muscarinic receptors to induction of fos and jun genes were investigated in neuroblastoma SH-SY5Y cells .
	manualset3
167904	5	412848	7	NULL	NULL	0	NULL	neuroblastoma SH-SY5Y cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The transduction pathways coupling muscarinic receptors to induction of fos and jun genes were investigated in neuroblastoma SH-SY5Y cells .
	manualset3
169605	6	412848	7	NULL	NULL	0	NULL	induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The transduction pathways coupling muscarinic receptors to induction of fos and jun genes were investigated in neuroblastoma SH-SY5Y cells .
	manualset3
167905	1	412849	7	NULL	NULL	0	NULL	 transferrin receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The transferrin receptor is often highly expressed in tumor cells whereas it is usually present at low levels in surrounding normal adult tissue .
	manualset3
167906	2	412849	7	NULL	NULL	0	NULL	tumor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The transferrin receptor is often highly expressed in tumor cells whereas it is usually present at low levels in surrounding normal adult tissue .
	manualset3
167907	3	412849	7	NULL	NULL	0	NULL	low levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The transferrin receptor is often highly expressed in tumor cells whereas it is usually present at low levels in surrounding normal adult tissue .
	manualset3
167908	4	412849	7	NULL	NULL	0	NULL	normal adult tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The transferrin receptor is often highly expressed in tumor cells whereas it is usually present at low levels in surrounding normal adult tissue .
	manualset3
167909	1	412850	7	NULL	NULL	0	NULL	transformer	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The transformer consists of solenoid-type coil and a magnetic core of ferrofluid , with the former fabricated by MEMS technology and the latter by a chemical co-precipitation method .
	manualset3
167910	2	412850	7	NULL	NULL	0	NULL	solenoid-type coil	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The transformer consists of solenoid-type coil and a magnetic core of ferrofluid , with the former fabricated by MEMS technology and the latter by a chemical co-precipitation method .
	manualset3
167911	3	412850	7	NULL	NULL	0	NULL	magnetic core of ferrofluid	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The transformer consists of solenoid-type coil and a magnetic core of ferrofluid , with the former fabricated by MEMS technology and the latter by a chemical co-precipitation method .
	manualset3
167912	4	412850	7	NULL	NULL	0	NULL	MEMS technology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The transformer consists of solenoid-type coil and a magnetic core of ferrofluid , with the former fabricated by MEMS technology and the latter by a chemical co-precipitation method .
	manualset3
167913	5	412850	7	NULL	NULL	0	NULL	chemical co-precipitation method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The transformer consists of solenoid-type coil and a magnetic core of ferrofluid , with the former fabricated by MEMS technology and the latter by a chemical co-precipitation method .
	manualset3
167914	1	412851	7	NULL	NULL	0	NULL	transgenic MT/bGH mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The transgenic MT/bGH mice had a marked hyperinsulinism without significant elevation of plasma glucose levels .
	manualset3
167915	2	412851	7	NULL	NULL	0	NULL	hyperinsulinism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The transgenic MT/bGH mice had a marked hyperinsulinism without significant elevation of plasma glucose levels .
	manualset3
167916	3	412851	7	NULL	NULL	0	NULL	elevation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The transgenic MT/bGH mice had a marked hyperinsulinism without significant elevation of plasma glucose levels .
	manualset3
167917	4	412851	7	NULL	NULL	0	NULL	plasma glucose levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The transgenic MT/bGH mice had a marked hyperinsulinism without significant elevation of plasma glucose levels .
	manualset3
167918	1	412852	7	NULL	NULL	0	NULL	 transient tritanopia	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The transient tritanopia and flicker fusion paradigms we used appear to be promising to investigate antiepileptic drugs with hitherto unknown modes of actions in human noninvasively .
	manualset3
167919	2	412852	7	NULL	NULL	0	NULL	flicker fusion paradigms	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The transient tritanopia and flicker fusion paradigms we used appear to be promising to investigate antiepileptic drugs with hitherto unknown modes of actions in human noninvasively .
	manualset3
167920	3	412852	7	NULL	NULL	0	NULL	antiepileptic drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The transient tritanopia and flicker fusion paradigms we used appear to be promising to investigate antiepileptic drugs with hitherto unknown modes of actions in human noninvasively .
	manualset3
167921	4	412852	7	NULL	NULL	0	NULL	modes of actions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The transient tritanopia and flicker fusion paradigms we used appear to be promising to investigate antiepileptic drugs with hitherto unknown modes of actions in human noninvasively .
	manualset3
167922	5	412852	7	NULL	NULL	0	NULL	human	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The transient tritanopia and flicker fusion paradigms we used appear to be promising to investigate antiepileptic drugs with hitherto unknown modes of actions in human noninvasively .
	manualset3
167923	1	412853	7	NULL	NULL	NULL	NULL	Acoustic and vibration background noise	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Acoustic and vibration background noise in the collapsed structure of the World Trade Center .
	manualset3
167924	2	412853	7	NULL	NULL	0	NULL	collapsed structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Acoustic and vibration background noise in the collapsed structure of the World Trade Center .
	manualset3
167925	3	412853	7	NULL	NULL	0	NULL	World Trade Center	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Acoustic and vibration background noise in the collapsed structure of the World Trade Center .
	manualset3
167926	1	412854	7	NULL	NULL	0	NULL	transition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The transition of SP ( CD45RC - ) thymocytes to fully mature CD45RC + CD4 T cells via intermediate peripheral RTE was accompanied at each stage by an increased ability of the maturing T cells to induce skin allograft rejection .
	manualset3
167927	2	412854	7	NULL	NULL	0	NULL	SP ( CD45RC - ) thymocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The transition of SP ( CD45RC - ) thymocytes to fully mature CD45RC + CD4 T cells via intermediate peripheral RTE was accompanied at each stage by an increased ability of the maturing T cells to induce skin allograft rejection .
	manualset3
167928	3	412854	7	NULL	NULL	0	NULL	fully mature CD45RC + CD4 T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The transition of SP ( CD45RC - ) thymocytes to fully mature CD45RC + CD4 T cells via intermediate peripheral RTE was accompanied at each stage by an increased ability of the maturing T cells to induce skin allograft rejection .
	manualset3
167929	4	412854	7	NULL	NULL	0	NULL	intermediate peripheral RTE	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The transition of SP ( CD45RC - ) thymocytes to fully mature CD45RC + CD4 T cells via intermediate peripheral RTE was accompanied at each stage by an increased ability of the maturing T cells to induce skin allograft rejection .
	manualset3
167930	5	412854	7	NULL	NULL	0	NULL	stage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The transition of SP ( CD45RC - ) thymocytes to fully mature CD45RC + CD4 T cells via intermediate peripheral RTE was accompanied at each stage by an increased ability of the maturing T cells to induce skin allograft rejection .
	manualset3
167931	6	412854	7	NULL	NULL	0	NULL	ability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The transition of SP ( CD45RC - ) thymocytes to fully mature CD45RC + CD4 T cells via intermediate peripheral RTE was accompanied at each stage by an increased ability of the maturing T cells to induce skin allograft rejection .
	manualset3
167932	7	412854	7	NULL	NULL	0	NULL	maturing T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The transition of SP ( CD45RC - ) thymocytes to fully mature CD45RC + CD4 T cells via intermediate peripheral RTE was accompanied at each stage by an increased ability of the maturing T cells to induce skin allograft rejection .
	manualset3
167933	8	412854	7	NULL	NULL	NULL	NULL	skin allograft rejection	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The transition of SP ( CD45RC - ) thymocytes to fully mature CD45RC + CD4 T cells via intermediate peripheral RTE was accompanied at each stage by an increased ability of the maturing T cells to induce skin allograft rejection .
	manualset3
167934	1	412855	7	NULL	NULL	NULL	NULL	transition	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The transition of hydrolase from blood into the bile is considered to be one of mechanisms of securing the enzyme homeostasis .
	manualset3
167935	2	412855	7	NULL	NULL	0	NULL	hydrolase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The transition of hydrolase from blood into the bile is considered to be one of mechanisms of securing the enzyme homeostasis .
	manualset3
167936	3	412855	7	NULL	NULL	0	NULL	blood 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The transition of hydrolase from blood into the bile is considered to be one of mechanisms of securing the enzyme homeostasis .
	manualset3
167937	4	412855	7	NULL	NULL	0	NULL	 bile 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The transition of hydrolase from blood into the bile is considered to be one of mechanisms of securing the enzyme homeostasis .
	manualset3
167938	5	412855	7	NULL	NULL	0	NULL	mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The transition of hydrolase from blood into the bile is considered to be one of mechanisms of securing the enzyme homeostasis .
	manualset3
167939	6	412855	7	NULL	NULL	0	NULL	enzyme homeostasis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The transition of hydrolase from blood into the bile is considered to be one of mechanisms of securing the enzyme homeostasis .
	manualset3
167940	1	412856	7	NULL	NULL	0	NULL	 translational attenuation regulatory model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The translational attenuation regulatory model suggests a mechanism that can explain the induction of cat-86 by chloramphenicol ( Cm ) .
	manualset3
167941	2	412856	7	NULL	NULL	0	NULL	mechanism 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The translational attenuation regulatory model suggests a mechanism that can explain the induction of cat-86 by chloramphenicol ( Cm ) .
	manualset3
167942	3	412856	7	NULL	NULL	0	NULL	induction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The translational attenuation regulatory model suggests a mechanism that can explain the induction of cat-86 by chloramphenicol ( Cm ) .
	manualset3
167943	4	412856	7	NULL	NULL	0	NULL	cat-86	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The translational attenuation regulatory model suggests a mechanism that can explain the induction of cat-86 by chloramphenicol ( Cm ) .
	manualset3
167944	5	412856	7	NULL	NULL	0	NULL	chloramphenicol ( Cm )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The translational attenuation regulatory model suggests a mechanism that can explain the induction of cat-86 by chloramphenicol ( Cm ) .
	manualset3
167945	1	412857	7	NULL	NULL	0	NULL	translocation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The translocation of protein kinase C betaII-green fluorescent protein to and from the plasma membrane in response to substance P indicates that the human SPR becomes activated within seconds of agonist exposure , and the response desensitizes within 30 s. This desensitization process coincides with a redistribution of GRK2 from the cytosol to the plasma membrane , followed by a robust redistribution of beta-arrestin 2 and a profound change in cell morphology that occurs after 1 min of SPR stimulation .
	manualset3
167946	2	412857	7	NULL	NULL	0	NULL	 protein kinase C betaII-green fluorescent protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The translocation of protein kinase C betaII-green fluorescent protein to and from the plasma membrane in response to substance P indicates that the human SPR becomes activated within seconds of agonist exposure , and the response desensitizes within 30 s. This desensitization process coincides with a redistribution of GRK2 from the cytosol to the plasma membrane , followed by a robust redistribution of beta-arrestin 2 and a profound change in cell morphology that occurs after 1 min of SPR stimulation .
	manualset3
167947	3	412857	7	NULL	NULL	0	NULL	plasma membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The translocation of protein kinase C betaII-green fluorescent protein to and from the plasma membrane in response to substance P indicates that the human SPR becomes activated within seconds of agonist exposure , and the response desensitizes within 30 s. This desensitization process coincides with a redistribution of GRK2 from the cytosol to the plasma membrane , followed by a robust redistribution of beta-arrestin 2 and a profound change in cell morphology that occurs after 1 min of SPR stimulation .
	manualset3
167948	4	412857	7	NULL	NULL	NULL	NULL	response	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The translocation of protein kinase C betaII-green fluorescent protein to and from the plasma membrane in response to substance P indicates that the human SPR becomes activated within seconds of agonist exposure , and the response desensitizes within 30 s. This desensitization process coincides with a redistribution of GRK2 from the cytosol to the plasma membrane , followed by a robust redistribution of beta-arrestin 2 and a profound change in cell morphology that occurs after 1 min of SPR stimulation .
	manualset3
167949	5	412857	7	NULL	NULL	0	NULL	substance P	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The translocation of protein kinase C betaII-green fluorescent protein to and from the plasma membrane in response to substance P indicates that the human SPR becomes activated within seconds of agonist exposure , and the response desensitizes within 30 s. This desensitization process coincides with a redistribution of GRK2 from the cytosol to the plasma membrane , followed by a robust redistribution of beta-arrestin 2 and a profound change in cell morphology that occurs after 1 min of SPR stimulation .
	manualset3
167950	6	412857	7	NULL	NULL	0	NULL	 human SPR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The translocation of protein kinase C betaII-green fluorescent protein to and from the plasma membrane in response to substance P indicates that the human SPR becomes activated within seconds of agonist exposure , and the response desensitizes within 30 s. This desensitization process coincides with a redistribution of GRK2 from the cytosol to the plasma membrane , followed by a robust redistribution of beta-arrestin 2 and a profound change in cell morphology that occurs after 1 min of SPR stimulation .
	manualset3
167951	7	412857	7	NULL	NULL	0	NULL	seconds	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The translocation of protein kinase C betaII-green fluorescent protein to and from the plasma membrane in response to substance P indicates that the human SPR becomes activated within seconds of agonist exposure , and the response desensitizes within 30 s. This desensitization process coincides with a redistribution of GRK2 from the cytosol to the plasma membrane , followed by a robust redistribution of beta-arrestin 2 and a profound change in cell morphology that occurs after 1 min of SPR stimulation .
	manualset3
167952	8	412857	7	NULL	NULL	NULL	NULL	agonist exposure	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The translocation of protein kinase C betaII-green fluorescent protein to and from the plasma membrane in response to substance P indicates that the human SPR becomes activated within seconds of agonist exposure , and the response desensitizes within 30 s. This desensitization process coincides with a redistribution of GRK2 from the cytosol to the plasma membrane , followed by a robust redistribution of beta-arrestin 2 and a profound change in cell morphology that occurs after 1 min of SPR stimulation .
	manualset3
167953	9	412857	7	NULL	NULL	NULL	NULL	response	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The translocation of protein kinase C betaII-green fluorescent protein to and from the plasma membrane in response to substance P indicates that the human SPR becomes activated within seconds of agonist exposure , and the response desensitizes within 30 s. This desensitization process coincides with a redistribution of GRK2 from the cytosol to the plasma membrane , followed by a robust redistribution of beta-arrestin 2 and a profound change in cell morphology that occurs after 1 min of SPR stimulation .
	manualset3
167954	10	412857	7	NULL	NULL	0	NULL	 30 s	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The translocation of protein kinase C betaII-green fluorescent protein to and from the plasma membrane in response to substance P indicates that the human SPR becomes activated within seconds of agonist exposure , and the response desensitizes within 30 s. This desensitization process coincides with a redistribution of GRK2 from the cytosol to the plasma membrane , followed by a robust redistribution of beta-arrestin 2 and a profound change in cell morphology that occurs after 1 min of SPR stimulation .
	manualset3
167955	11	412857	7	NULL	NULL	0	NULL	desensitization process	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The translocation of protein kinase C betaII-green fluorescent protein to and from the plasma membrane in response to substance P indicates that the human SPR becomes activated within seconds of agonist exposure , and the response desensitizes within 30 s. This desensitization process coincides with a redistribution of GRK2 from the cytosol to the plasma membrane , followed by a robust redistribution of beta-arrestin 2 and a profound change in cell morphology that occurs after 1 min of SPR stimulation .
	manualset3
167956	12	412857	7	NULL	NULL	0	NULL	 redistribution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The translocation of protein kinase C betaII-green fluorescent protein to and from the plasma membrane in response to substance P indicates that the human SPR becomes activated within seconds of agonist exposure , and the response desensitizes within 30 s. This desensitization process coincides with a redistribution of GRK2 from the cytosol to the plasma membrane , followed by a robust redistribution of beta-arrestin 2 and a profound change in cell morphology that occurs after 1 min of SPR stimulation .
	manualset3
167957	13	412857	7	NULL	NULL	0	NULL	GRK2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The translocation of protein kinase C betaII-green fluorescent protein to and from the plasma membrane in response to substance P indicates that the human SPR becomes activated within seconds of agonist exposure , and the response desensitizes within 30 s. This desensitization process coincides with a redistribution of GRK2 from the cytosol to the plasma membrane , followed by a robust redistribution of beta-arrestin 2 and a profound change in cell morphology that occurs after 1 min of SPR stimulation .
	manualset3
167958	14	412857	7	NULL	NULL	0	NULL	cytosol	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The translocation of protein kinase C betaII-green fluorescent protein to and from the plasma membrane in response to substance P indicates that the human SPR becomes activated within seconds of agonist exposure , and the response desensitizes within 30 s. This desensitization process coincides with a redistribution of GRK2 from the cytosol to the plasma membrane , followed by a robust redistribution of beta-arrestin 2 and a profound change in cell morphology that occurs after 1 min of SPR stimulation .
	manualset3
167959	15	412857	7	NULL	NULL	0	NULL	plasma membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The translocation of protein kinase C betaII-green fluorescent protein to and from the plasma membrane in response to substance P indicates that the human SPR becomes activated within seconds of agonist exposure , and the response desensitizes within 30 s. This desensitization process coincides with a redistribution of GRK2 from the cytosol to the plasma membrane , followed by a robust redistribution of beta-arrestin 2 and a profound change in cell morphology that occurs after 1 min of SPR stimulation .
	manualset3
167960	16	412857	7	NULL	NULL	0	NULL	 redistribution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The translocation of protein kinase C betaII-green fluorescent protein to and from the plasma membrane in response to substance P indicates that the human SPR becomes activated within seconds of agonist exposure , and the response desensitizes within 30 s. This desensitization process coincides with a redistribution of GRK2 from the cytosol to the plasma membrane , followed by a robust redistribution of beta-arrestin 2 and a profound change in cell morphology that occurs after 1 min of SPR stimulation .
	manualset3
167961	17	412857	7	NULL	NULL	0	NULL	beta-arrestin 2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The translocation of protein kinase C betaII-green fluorescent protein to and from the plasma membrane in response to substance P indicates that the human SPR becomes activated within seconds of agonist exposure , and the response desensitizes within 30 s. This desensitization process coincides with a redistribution of GRK2 from the cytosol to the plasma membrane , followed by a robust redistribution of beta-arrestin 2 and a profound change in cell morphology that occurs after 1 min of SPR stimulation .
	manualset3
167962	18	412857	7	NULL	NULL	NULL	NULL	cell morphology	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The translocation of protein kinase C betaII-green fluorescent protein to and from the plasma membrane in response to substance P indicates that the human SPR becomes activated within seconds of agonist exposure , and the response desensitizes within 30 s. This desensitization process coincides with a redistribution of GRK2 from the cytosol to the plasma membrane , followed by a robust redistribution of beta-arrestin 2 and a profound change in cell morphology that occurs after 1 min of SPR stimulation .
	manualset3
167963	19	412857	7	NULL	NULL	0	NULL	1 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The translocation of protein kinase C betaII-green fluorescent protein to and from the plasma membrane in response to substance P indicates that the human SPR becomes activated within seconds of agonist exposure , and the response desensitizes within 30 s. This desensitization process coincides with a redistribution of GRK2 from the cytosol to the plasma membrane , followed by a robust redistribution of beta-arrestin 2 and a profound change in cell morphology that occurs after 1 min of SPR stimulation .
	manualset3
167964	20	412857	7	NULL	NULL	0	NULL	SPR stimulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The translocation of protein kinase C betaII-green fluorescent protein to and from the plasma membrane in response to substance P indicates that the human SPR becomes activated within seconds of agonist exposure , and the response desensitizes within 30 s. This desensitization process coincides with a redistribution of GRK2 from the cytosol to the plasma membrane , followed by a robust redistribution of beta-arrestin 2 and a profound change in cell morphology that occurs after 1 min of SPR stimulation .
	manualset3
169639	21	412857	7	NULL	NULL	NULL	NULL	change	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The translocation of protein kinase C betaII-green fluorescent protein to and from the plasma membrane in response to substance P indicates that the human SPR becomes activated within seconds of agonist exposure , and the response desensitizes within 30 s. This desensitization process coincides with a redistribution of GRK2 from the cytosol to the plasma membrane , followed by a robust redistribution of beta-arrestin 2 and a profound change in cell morphology that occurs after 1 min of SPR stimulation .
	manualset3
167965	1	412858	7	NULL	NULL	0	NULL	translocons	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The translocons at the outer envelope membrane of chloroplasts ( TOCs ) initiate the import of thousands of nucleus-encoded proteins into the organelle .
	manualset3
167966	2	412858	7	NULL	NULL	0	NULL	outer envelope membrane of chloroplasts ( TOCs )	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The translocons at the outer envelope membrane of chloroplasts ( TOCs ) initiate the import of thousands of nucleus-encoded proteins into the organelle .
	manualset3
167967	3	412858	7	NULL	NULL	0	NULL	import 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The translocons at the outer envelope membrane of chloroplasts ( TOCs ) initiate the import of thousands of nucleus-encoded proteins into the organelle .
	manualset3
167968	4	412858	7	NULL	NULL	0	NULL	thousands	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The translocons at the outer envelope membrane of chloroplasts ( TOCs ) initiate the import of thousands of nucleus-encoded proteins into the organelle .
	manualset3
167969	5	412858	7	NULL	NULL	0	NULL	nucleus-encoded proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The translocons at the outer envelope membrane of chloroplasts ( TOCs ) initiate the import of thousands of nucleus-encoded proteins into the organelle .
	manualset3
167970	6	412858	7	NULL	NULL	0	NULL	organelle	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The translocons at the outer envelope membrane of chloroplasts ( TOCs ) initiate the import of thousands of nucleus-encoded proteins into the organelle .
	manualset3
167971	1	412859	7	NULL	NULL	0	NULL	transmembrane permeability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The transmembrane permeability of DEET and oxybenzone across piglet skin and PDMS membrane was dependent on dissolving vehicles and test concentrations .
	manualset3
167972	2	412859	7	NULL	NULL	0	NULL	DEET	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The transmembrane permeability of DEET and oxybenzone across piglet skin and PDMS membrane was dependent on dissolving vehicles and test concentrations .
	manualset3
167973	3	412859	7	NULL	NULL	0	NULL	oxybenzone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The transmembrane permeability of DEET and oxybenzone across piglet skin and PDMS membrane was dependent on dissolving vehicles and test concentrations .
	manualset3
167974	4	412859	7	NULL	NULL	NULL	NULL	piglet skin	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The transmembrane permeability of DEET and oxybenzone across piglet skin and PDMS membrane was dependent on dissolving vehicles and test concentrations .
	manualset3
167975	5	412859	7	NULL	NULL	0	NULL	PDMS membrane	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The transmembrane permeability of DEET and oxybenzone across piglet skin and PDMS membrane was dependent on dissolving vehicles and test concentrations .
	manualset3
167976	6	412859	7	NULL	NULL	0	NULL	dissolving vehicles 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The transmembrane permeability of DEET and oxybenzone across piglet skin and PDMS membrane was dependent on dissolving vehicles and test concentrations .
	manualset3
167977	7	412859	7	NULL	NULL	0	NULL	test concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The transmembrane permeability of DEET and oxybenzone across piglet skin and PDMS membrane was dependent on dissolving vehicles and test concentrations .
	manualset3
167978	1	412860	7	NULL	NULL	0	NULL	transmembrane DNA-binding protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The transmembrane DNA-binding protein , ToxR , of Vibrio cholerae is a global transcriptional regulator of virulence gene expression .
	manualset3
167979	2	412860	7	NULL	NULL	0	NULL	ToxR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The transmembrane DNA-binding protein , ToxR , of Vibrio cholerae is a global transcriptional regulator of virulence gene expression .
	manualset3
167980	3	412860	7	NULL	NULL	0	NULL	Vibrio cholerae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The transmembrane DNA-binding protein , ToxR , of Vibrio cholerae is a global transcriptional regulator of virulence gene expression .
	manualset3
167981	4	412860	7	NULL	NULL	0	NULL	global transcriptional regulator	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The transmembrane DNA-binding protein , ToxR , of Vibrio cholerae is a global transcriptional regulator of virulence gene expression .
	manualset3
167982	5	412860	7	NULL	NULL	0	NULL	virulence gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The transmembrane DNA-binding protein , ToxR , of Vibrio cholerae is a global transcriptional regulator of virulence gene expression .
	manualset3
167983	1	412861	7	NULL	NULL	0	NULL	transmission area	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The transmission area of this disease continues to expand due to many direct and indirect factors linked to urban sprawl , increased travel and global warming .
	manualset3
167984	2	412861	7	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The transmission area of this disease continues to expand due to many direct and indirect factors linked to urban sprawl , increased travel and global warming .
	manualset3
167985	3	412861	7	NULL	NULL	0	NULL	 direct factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The transmission area of this disease continues to expand due to many direct and indirect factors linked to urban sprawl , increased travel and global warming .
	manualset3
167986	4	412861	7	NULL	NULL	0	NULL	indirect factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The transmission area of this disease continues to expand due to many direct and indirect factors linked to urban sprawl , increased travel and global warming .
	manualset3
167987	5	412861	7	NULL	NULL	0	NULL	urban sprawl	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The transmission area of this disease continues to expand due to many direct and indirect factors linked to urban sprawl , increased travel and global warming .
	manualset3
167988	6	412861	7	NULL	NULL	0	NULL	increased travel 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The transmission area of this disease continues to expand due to many direct and indirect factors linked to urban sprawl , increased travel and global warming .
	manualset3
167989	7	412861	7	NULL	NULL	0	NULL	global warming	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The transmission area of this disease continues to expand due to many direct and indirect factors linked to urban sprawl , increased travel and global warming .
	manualset3
167990	1	412862	7	NULL	NULL	0	NULL	transmission	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The transmission is either transfusional or nosocomial .
	manualset3
167993	1	412863	7	NULL	NULL	0	NULL	transplantable islet-cell tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The transplantable islet-cell tumor of the golden hamster has already been shown to produce hypoglycemia and hyperinsulinemia in the receptor animal .
	manualset3
167994	2	412863	7	NULL	NULL	0	NULL	golden hamster	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The transplantable islet-cell tumor of the golden hamster has already been shown to produce hypoglycemia and hyperinsulinemia in the receptor animal .
	manualset3
167995	3	412863	7	NULL	NULL	0	NULL	hypoglycemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The transplantable islet-cell tumor of the golden hamster has already been shown to produce hypoglycemia and hyperinsulinemia in the receptor animal .
	manualset3
167996	4	412863	7	NULL	NULL	0	NULL	hyperinsulinemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The transplantable islet-cell tumor of the golden hamster has already been shown to produce hypoglycemia and hyperinsulinemia in the receptor animal .
	manualset3
167997	5	412863	7	NULL	NULL	0	NULL	receptor animal	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The transplantable islet-cell tumor of the golden hamster has already been shown to produce hypoglycemia and hyperinsulinemia in the receptor animal .
	manualset3
167998	1	412864	7	NULL	NULL	0	NULL	Acoustic rhinometry	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Acoustic rhinometry and lavage biomarkers in relation to some building characteristics in Swedish schools .
	manualset3
167999	2	412864	7	NULL	NULL	0	NULL	lavage biomarkers	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Acoustic rhinometry and lavage biomarkers in relation to some building characteristics in Swedish schools .
	manualset3
168000	3	412864	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Acoustic rhinometry and lavage biomarkers in relation to some building characteristics in Swedish schools .
	manualset3
168001	4	412864	7	NULL	NULL	NULL	NULL	 building characteristics	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Acoustic rhinometry and lavage biomarkers in relation to some building characteristics in Swedish schools .
	manualset3
168002	5	412864	7	NULL	NULL	0	NULL	Swedish schools	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Acoustic rhinometry and lavage biomarkers in relation to some building characteristics in Swedish schools .
	manualset3
168003	1	412865	7	NULL	NULL	0	NULL	transport 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The transport of glucose across the blood-brain barrier ( BBB ) is mediated by the high molecular mass ( 55-kDa ) isoform of the GLUT1 glucose transporter protein .
	manualset3
168004	2	412865	7	NULL	NULL	0	NULL	glucose	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The transport of glucose across the blood-brain barrier ( BBB ) is mediated by the high molecular mass ( 55-kDa ) isoform of the GLUT1 glucose transporter protein .
	manualset3
168005	3	412865	7	NULL	NULL	0	NULL	blood-brain barrier ( BBB )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The transport of glucose across the blood-brain barrier ( BBB ) is mediated by the high molecular mass ( 55-kDa ) isoform of the GLUT1 glucose transporter protein .
	manualset3
168006	4	412865	7	NULL	NULL	0	NULL	high molecular mass isoform	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The transport of glucose across the blood-brain barrier ( BBB ) is mediated by the high molecular mass ( 55-kDa ) isoform of the GLUT1 glucose transporter protein .
	manualset3
168007	5	412865	7	NULL	NULL	0	NULL	 55-kDa	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The transport of glucose across the blood-brain barrier ( BBB ) is mediated by the high molecular mass ( 55-kDa ) isoform of the GLUT1 glucose transporter protein .
	manualset3
168008	6	412865	7	NULL	NULL	0	NULL	GLUT1 glucose transporter protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The transport of glucose across the blood-brain barrier ( BBB ) is mediated by the high molecular mass ( 55-kDa ) isoform of the GLUT1 glucose transporter protein .
	manualset3
168009	1	412866	7	NULL	NULL	NULL	NULL	transport of proteins	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The transport of proteins into the nucleus proceeds via the cytosol of a cell , therefore , ammodytoxin passed the cytosol of the neuron on its way to the nucleus .
	manualset3
168010	2	412866	7	NULL	NULL	0	NULL	 nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The transport of proteins into the nucleus proceeds via the cytosol of a cell , therefore , ammodytoxin passed the cytosol of the neuron on its way to the nucleus .
	manualset3
168011	3	412866	7	NULL	NULL	0	NULL	cytosol	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The transport of proteins into the nucleus proceeds via the cytosol of a cell , therefore , ammodytoxin passed the cytosol of the neuron on its way to the nucleus .
	manualset3
168012	4	412866	7	NULL	NULL	0	NULL	cell 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The transport of proteins into the nucleus proceeds via the cytosol of a cell , therefore , ammodytoxin passed the cytosol of the neuron on its way to the nucleus .
	manualset3
168013	5	412866	7	NULL	NULL	0	NULL	ammodytoxin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The transport of proteins into the nucleus proceeds via the cytosol of a cell , therefore , ammodytoxin passed the cytosol of the neuron on its way to the nucleus .
	manualset3
168014	6	412866	7	NULL	NULL	0	NULL	cytosol	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The transport of proteins into the nucleus proceeds via the cytosol of a cell , therefore , ammodytoxin passed the cytosol of the neuron on its way to the nucleus .
	manualset3
168015	7	412866	7	NULL	NULL	0	NULL	neuron	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The transport of proteins into the nucleus proceeds via the cytosol of a cell , therefore , ammodytoxin passed the cytosol of the neuron on its way to the nucleus .
	manualset3
168016	8	412866	7	NULL	NULL	0	NULL	nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The transport of proteins into the nucleus proceeds via the cytosol of a cell , therefore , ammodytoxin passed the cytosol of the neuron on its way to the nucleus .
	manualset3
168017	1	412867	7	NULL	NULL	0	NULL	treating physician	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The treating physician revealed the diagnosis to the family first , and then told the patient : `` You do n't have any cancer yet , but if we do n't treat you , it will progress to a cancer '' .
	manualset3
168018	2	412867	7	NULL	NULL	0	NULL	diagnosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The treating physician revealed the diagnosis to the family first , and then told the patient : `` You do n't have any cancer yet , but if we do n't treat you , it will progress to a cancer '' .
	manualset3
168019	3	412867	7	NULL	NULL	0	NULL	family	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The treating physician revealed the diagnosis to the family first , and then told the patient : `` You do n't have any cancer yet , but if we do n't treat you , it will progress to a cancer '' .
	manualset3
168020	4	412867	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The treating physician revealed the diagnosis to the family first , and then told the patient : `` You do n't have any cancer yet , but if we do n't treat you , it will progress to a cancer '' .
	manualset3
168021	5	412867	7	NULL	NULL	0	NULL	 `` You do n't have any cancer yet , but if we do n't treat you , it will progress to a cancer '' 	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	The treating physician revealed the diagnosis to the family first , and then told the patient : `` You do n't have any cancer yet , but if we do n't treat you , it will progress to a cancer '' .
	manualset3
168022	1	412868	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of acute leukemia with the folic acid antagonist , aminopterin .
	manualset3
168023	2	412868	7	NULL	NULL	NULL	NULL	acute leukemia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The treatment of acute leukemia with the folic acid antagonist , aminopterin .
	manualset3
168024	3	412868	7	NULL	NULL	NULL	NULL	folic acid antagonist	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The treatment of acute leukemia with the folic acid antagonist , aminopterin .
	manualset3
168025	4	412868	7	NULL	NULL	NULL	NULL	aminopterin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The treatment of acute leukemia with the folic acid antagonist , aminopterin .
	manualset3
168026	1	412869	7	NULL	NULL	0	NULL	 treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of carcinoma of the cervix by continuous intra-arterial methotrexate and by intermittent intramuscular leucovorin .
	manualset3
168027	2	412869	7	NULL	NULL	0	NULL	carcinoma of the cervix	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of carcinoma of the cervix by continuous intra-arterial methotrexate and by intermittent intramuscular leucovorin .
	manualset3
168028	3	412869	7	NULL	NULL	0	NULL	continuous intra-arterial methotrexate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of carcinoma of the cervix by continuous intra-arterial methotrexate and by intermittent intramuscular leucovorin .
	manualset3
168029	4	412869	7	NULL	NULL	0	NULL	intermittent intramuscular leucovorin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of carcinoma of the cervix by continuous intra-arterial methotrexate and by intermittent intramuscular leucovorin .
	manualset3
168030	1	412870	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of cardiac arrest .
	manualset3
168031	2	412870	7	NULL	NULL	0	NULL	cardiac arrest	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of cardiac arrest .
	manualset3
168032	1	412871	7	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of choroidal neovascular membranes by alpha interferon .
	manualset3
168033	2	412871	7	NULL	NULL	0	NULL	choroidal neovascular membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of choroidal neovascular membranes by alpha interferon .
	manualset3
168034	3	412871	7	NULL	NULL	0	NULL	alpha interferon	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of choroidal neovascular membranes by alpha interferon .
	manualset3
168035	1	412872	7	NULL	NULL	0	NULL	 treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of human salivary gland epithelial cells ( SGECs ) with SS anti-Ro/SSA autoantibodies ( Abs ) result in a progressive increase in NF-B-DNA binding , that includes a marked enhancement in NF-B subunit p65 protein-DNA binding .
	manualset3
168036	2	412872	7	NULL	NULL	0	NULL	human salivary gland epithelial cells ( SGECs )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of human salivary gland epithelial cells ( SGECs ) with SS anti-Ro/SSA autoantibodies ( Abs ) result in a progressive increase in NF-B-DNA binding , that includes a marked enhancement in NF-B subunit p65 protein-DNA binding .
	manualset3
168037	3	412872	7	NULL	NULL	NULL	NULL	SS anti-Ro/SSA autoantibodies ( Abs ) 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The treatment of human salivary gland epithelial cells ( SGECs ) with SS anti-Ro/SSA autoantibodies ( Abs ) result in a progressive increase in NF-B-DNA binding , that includes a marked enhancement in NF-B subunit p65 protein-DNA binding .
	manualset3
168038	4	412872	7	NULL	NULL	NULL	NULL	progressive increase	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The treatment of human salivary gland epithelial cells ( SGECs ) with SS anti-Ro/SSA autoantibodies ( Abs ) result in a progressive increase in NF-B-DNA binding , that includes a marked enhancement in NF-B subunit p65 protein-DNA binding .
	manualset3
168039	5	412872	7	NULL	NULL	0	NULL	NF-B-DNA binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of human salivary gland epithelial cells ( SGECs ) with SS anti-Ro/SSA autoantibodies ( Abs ) result in a progressive increase in NF-B-DNA binding , that includes a marked enhancement in NF-B subunit p65 protein-DNA binding .
	manualset3
168040	6	412872	7	NULL	NULL	0	NULL	NF-B subunit p65 protein-DNA binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of human salivary gland epithelial cells ( SGECs ) with SS anti-Ro/SSA autoantibodies ( Abs ) result in a progressive increase in NF-B-DNA binding , that includes a marked enhancement in NF-B subunit p65 protein-DNA binding .
	manualset3
169650	7	412872	7	NULL	NULL	0	NULL	marked enhancement 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of human salivary gland epithelial cells ( SGECs ) with SS anti-Ro/SSA autoantibodies ( Abs ) result in a progressive increase in NF-B-DNA binding , that includes a marked enhancement in NF-B subunit p65 protein-DNA binding .
	manualset3
168041	1	412873	7	NULL	NULL	0	NULL	Acquired ileal diverticulum	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acquired ileal diverticulum is an uncommon condition and diagnosis is often difficult when bleeding occurs from this source .
	manualset3
168042	2	412873	7	NULL	NULL	0	NULL	 uncommon condition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acquired ileal diverticulum is an uncommon condition and diagnosis is often difficult when bleeding occurs from this source .
	manualset3
168043	3	412873	7	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acquired ileal diverticulum is an uncommon condition and diagnosis is often difficult when bleeding occurs from this source .
	manualset3
168044	4	412873	7	NULL	NULL	0	NULL	bleeding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acquired ileal diverticulum is an uncommon condition and diagnosis is often difficult when bleeding occurs from this source .
	manualset3
168045	5	412873	7	NULL	NULL	0	NULL	source	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Acquired ileal diverticulum is an uncommon condition and diagnosis is often difficult when bleeding occurs from this source .
	manualset3
168046	1	412874	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of induced immune deficiency with interleukin-2 .
	manualset3
168047	2	412874	7	NULL	NULL	0	NULL	induced immune deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of induced immune deficiency with interleukin-2 .
	manualset3
168048	3	412874	7	NULL	NULL	0	NULL	interleukin-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of induced immune deficiency with interleukin-2 .
	manualset3
168049	1	412875	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of iris melanoma .
	manualset3
168050	2	412875	7	NULL	NULL	0	NULL	iris melanoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of iris melanoma .
	manualset3
168051	1	412876	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of recombinant TNF-alpha to HL-60 cells resulted in the increased PLD activity as determined by the phosphatidylethanol formation in the presence of 1 % ethanol .
	manualset3
168052	2	412876	7	NULL	NULL	0	NULL	recombinant TNF-alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of recombinant TNF-alpha to HL-60 cells resulted in the increased PLD activity as determined by the phosphatidylethanol formation in the presence of 1 % ethanol .
	manualset3
168053	3	412876	7	NULL	NULL	0	NULL	HL-60 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of recombinant TNF-alpha to HL-60 cells resulted in the increased PLD activity as determined by the phosphatidylethanol formation in the presence of 1 % ethanol .
	manualset3
168054	4	412876	7	NULL	NULL	0	NULL	 increased PLD activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of recombinant TNF-alpha to HL-60 cells resulted in the increased PLD activity as determined by the phosphatidylethanol formation in the presence of 1 % ethanol .
	manualset3
168055	5	412876	7	NULL	NULL	0	NULL	phosphatidylethanol formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of recombinant TNF-alpha to HL-60 cells resulted in the increased PLD activity as determined by the phosphatidylethanol formation in the presence of 1 % ethanol .
	manualset3
168056	6	412876	7	NULL	NULL	0	NULL	presence	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of recombinant TNF-alpha to HL-60 cells resulted in the increased PLD activity as determined by the phosphatidylethanol formation in the presence of 1 % ethanol .
	manualset3
168057	7	412876	7	NULL	NULL	0	NULL	 1 % ethanol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of recombinant TNF-alpha to HL-60 cells resulted in the increased PLD activity as determined by the phosphatidylethanol formation in the presence of 1 % ethanol .
	manualset3
168058	1	412877	7	NULL	NULL	0	NULL	 treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of the enzymes in vitro by ethanolamine exhibited a reversible inhibition of the mixed and competitive types for alpha-glucosidase and beta-glucuronidase , respectively .
	manualset3
168059	2	412877	7	NULL	NULL	NULL	NULL	enzymes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The treatment of the enzymes in vitro by ethanolamine exhibited a reversible inhibition of the mixed and competitive types for alpha-glucosidase and beta-glucuronidase , respectively .
	manualset3
168060	3	412877	7	NULL	NULL	0	NULL	ethanolamine	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of the enzymes in vitro by ethanolamine exhibited a reversible inhibition of the mixed and competitive types for alpha-glucosidase and beta-glucuronidase , respectively .
	manualset3
168061	4	412877	7	NULL	NULL	0	NULL	reversible inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of the enzymes in vitro by ethanolamine exhibited a reversible inhibition of the mixed and competitive types for alpha-glucosidase and beta-glucuronidase , respectively .
	manualset3
168062	5	412877	7	NULL	NULL	NULL	NULL	mixed types	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The treatment of the enzymes in vitro by ethanolamine exhibited a reversible inhibition of the mixed and competitive types for alpha-glucosidase and beta-glucuronidase , respectively .
	manualset3
168063	6	412877	7	NULL	NULL	NULL	NULL	competitive types	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The treatment of the enzymes in vitro by ethanolamine exhibited a reversible inhibition of the mixed and competitive types for alpha-glucosidase and beta-glucuronidase , respectively .
	manualset3
168064	7	412877	7	NULL	NULL	0	NULL	alpha-glucosidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of the enzymes in vitro by ethanolamine exhibited a reversible inhibition of the mixed and competitive types for alpha-glucosidase and beta-glucuronidase , respectively .
	manualset3
168065	8	412877	7	NULL	NULL	0	NULL	beta-glucuronidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of the enzymes in vitro by ethanolamine exhibited a reversible inhibition of the mixed and competitive types for alpha-glucosidase and beta-glucuronidase , respectively .
	manualset3
168066	1	412878	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment with acetaminophen and Cd lasted 2 and 10 months , respectively .
	manualset3
168067	2	412878	7	NULL	NULL	0	NULL	acetaminophen	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment with acetaminophen and Cd lasted 2 and 10 months , respectively .
	manualset3
168068	3	412878	7	NULL	NULL	0	NULL	 Cd	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment with acetaminophen and Cd lasted 2 and 10 months , respectively .
	manualset3
168069	4	412878	7	NULL	NULL	0	NULL	2 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment with acetaminophen and Cd lasted 2 and 10 months , respectively .
	manualset3
168070	5	412878	7	NULL	NULL	0	NULL	10 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment with acetaminophen and Cd lasted 2 and 10 months , respectively .
	manualset3
168071	1	412879	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment with pergolide in these cases might be more beneficial than with short-acting PDE-5 inhibitor sildenafile .
	manualset3
168072	2	412879	7	NULL	NULL	NULL	NULL	pergolide	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The treatment with pergolide in these cases might be more beneficial than with short-acting PDE-5 inhibitor sildenafile .
	manualset3
168073	3	412879	7	NULL	NULL	0	NULL	cases	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment with pergolide in these cases might be more beneficial than with short-acting PDE-5 inhibitor sildenafile .
	manualset3
168074	4	412879	7	NULL	NULL	NULL	NULL	short-acting PDE-5 inhibitor	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The treatment with pergolide in these cases might be more beneficial than with short-acting PDE-5 inhibitor sildenafile .
	manualset3
168075	5	412879	7	NULL	NULL	NULL	NULL	sildenafile	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The treatment with pergolide in these cases might be more beneficial than with short-acting PDE-5 inhibitor sildenafile .
	manualset3
168076	1	412880	7	NULL	NULL	0	NULL	trees	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The trees derived from Bayesian , ML , and NJ analyses were topologically identical to the MP analysis except for the position of P. mystaceus .
	manualset3
168077	2	412880	7	NULL	NULL	0	NULL	Bayesian analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The trees derived from Bayesian , ML , and NJ analyses were topologically identical to the MP analysis except for the position of P. mystaceus .
	manualset3
168078	3	412880	7	NULL	NULL	0	NULL	ML analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The trees derived from Bayesian , ML , and NJ analyses were topologically identical to the MP analysis except for the position of P. mystaceus .
	manualset3
168079	4	412880	7	NULL	NULL	0	NULL	NJ analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The trees derived from Bayesian , ML , and NJ analyses were topologically identical to the MP analysis except for the position of P. mystaceus .
	manualset3
168080	5	412880	7	NULL	NULL	0	NULL	MP analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The trees derived from Bayesian , ML , and NJ analyses were topologically identical to the MP analysis except for the position of P. mystaceus .
	manualset3
168081	6	412880	7	NULL	NULL	0	NULL	position	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The trees derived from Bayesian , ML , and NJ analyses were topologically identical to the MP analysis except for the position of P. mystaceus .
	manualset3
168082	7	412880	7	NULL	NULL	0	NULL	P. mystaceus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The trees derived from Bayesian , ML , and NJ analyses were topologically identical to the MP analysis except for the position of P. mystaceus .
	manualset3
168083	1	412881	7	NULL	NULL	0	NULL	 trend	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The trend is towards less aggressive , outpatient schedules of chemotherapy .
	manualset3
168084	2	412881	7	NULL	NULL	0	NULL	outpatient schedules	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The trend is towards less aggressive , outpatient schedules of chemotherapy .
	manualset3
168085	3	412881	7	NULL	NULL	0	NULL	chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The trend is towards less aggressive , outpatient schedules of chemotherapy .
	manualset3
168086	1	412882	7	NULL	NULL	0	NULL	Acquired intolerance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Acquired intolerance to solvents following pesticide/solvent exposure in a building : a new group of workers at risk for multiple chemical sensitivities ?
	manualset3
168087	2	412882	7	NULL	NULL	0	NULL	solvents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Acquired intolerance to solvents following pesticide/solvent exposure in a building : a new group of workers at risk for multiple chemical sensitivities ?
	manualset3
168088	3	412882	7	NULL	NULL	0	NULL	pesticide/solvent exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Acquired intolerance to solvents following pesticide/solvent exposure in a building : a new group of workers at risk for multiple chemical sensitivities ?
	manualset3
168089	4	412882	7	NULL	NULL	0	NULL	building	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Acquired intolerance to solvents following pesticide/solvent exposure in a building : a new group of workers at risk for multiple chemical sensitivities ?
	manualset3
168090	5	412882	7	NULL	NULL	0	NULL	new group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Acquired intolerance to solvents following pesticide/solvent exposure in a building : a new group of workers at risk for multiple chemical sensitivities ?
	manualset3
168091	6	412882	7	NULL	NULL	0	NULL	workers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Acquired intolerance to solvents following pesticide/solvent exposure in a building : a new group of workers at risk for multiple chemical sensitivities ?
	manualset3
168092	7	412882	7	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acquired intolerance to solvents following pesticide/solvent exposure in a building : a new group of workers at risk for multiple chemical sensitivities ?
	manualset3
168093	8	412882	7	NULL	NULL	0	NULL	multiple chemical sensitivities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acquired intolerance to solvents following pesticide/solvent exposure in a building : a new group of workers at risk for multiple chemical sensitivities ?
	manualset3
168094	1	412883	7	NULL	NULL	0	NULL	trends 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The trends in the measured BDEs suggest two very different binding modes for the Na ( + ) ( xBA ) complexes , while theory finds four .
	manualset3
168095	2	412883	7	NULL	NULL	0	NULL	 measured BDEs	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The trends in the measured BDEs suggest two very different binding modes for the Na ( + ) ( xBA ) complexes , while theory finds four .
	manualset3
168096	3	412883	7	NULL	NULL	0	NULL	 two 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The trends in the measured BDEs suggest two very different binding modes for the Na ( + ) ( xBA ) complexes , while theory finds four .
	manualset3
168097	4	412883	7	NULL	NULL	0	NULL	binding modes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The trends in the measured BDEs suggest two very different binding modes for the Na ( + ) ( xBA ) complexes , while theory finds four .
	manualset3
168098	5	412883	7	NULL	NULL	0	NULL	Na ( + ) ( xBA ) complexes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The trends in the measured BDEs suggest two very different binding modes for the Na ( + ) ( xBA ) complexes , while theory finds four .
	manualset3
168099	6	412883	7	NULL	NULL	0	NULL	theory	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The trends in the measured BDEs suggest two very different binding modes for the Na ( + ) ( xBA ) complexes , while theory finds four .
	manualset3
168100	7	412883	7	NULL	NULL	0	NULL	four	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The trends in the measured BDEs suggest two very different binding modes for the Na ( + ) ( xBA ) complexes , while theory finds four .
	manualset3
168101	1	412884	7	NULL	NULL	0	NULL	trial court	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The trial court declined to make a temporary child support order because it found that the unborn child was not yet a `` child of the marriage '' under state law .
	manualset3
168102	2	412884	7	NULL	NULL	0	NULL	temporary child support order	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The trial court declined to make a temporary child support order because it found that the unborn child was not yet a `` child of the marriage '' under state law .
	manualset3
168103	3	412884	7	NULL	NULL	NULL	NULL	unborn child 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The trial court declined to make a temporary child support order because it found that the unborn child was not yet a `` child of the marriage '' under state law .
	manualset3
168104	4	412884	7	NULL	NULL	0	NULL	`` child of the marriage ''	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The trial court declined to make a temporary child support order because it found that the unborn child was not yet a `` child of the marriage '' under state law .
	manualset3
168105	5	412884	7	NULL	NULL	0	NULL	state law	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The trial court declined to make a temporary child support order because it found that the unborn child was not yet a `` child of the marriage '' under state law .
	manualset3
168106	1	412885	7	NULL	NULL	0	NULL	triangular profile	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The triangular profile of Talbot interferometric fringes has been recorded using a CCD and computer system .
	manualset3
168107	2	412885	7	NULL	NULL	0	NULL	Talbot interferometric fringes	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The triangular profile of Talbot interferometric fringes has been recorded using a CCD and computer system .
	manualset3
168108	3	412885	7	NULL	NULL	0	NULL	 CCD	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The triangular profile of Talbot interferometric fringes has been recorded using a CCD and computer system .
	manualset3
168109	4	412885	7	NULL	NULL	0	NULL	computer system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The triangular profile of Talbot interferometric fringes has been recorded using a CCD and computer system .
	manualset3
168110	1	412886	7	NULL	NULL	0	NULL	tripartite leader sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The tripartite leader sequence of human adenovirus mRNA linked with a major late promoter enhancer gave the most universal and highest enhancement of gene expression levels .
	manualset3
168111	2	412886	7	NULL	NULL	0	NULL	human adenovirus mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The tripartite leader sequence of human adenovirus mRNA linked with a major late promoter enhancer gave the most universal and highest enhancement of gene expression levels .
	manualset3
168112	3	412886	7	NULL	NULL	0	NULL	major late promoter enhancer	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The tripartite leader sequence of human adenovirus mRNA linked with a major late promoter enhancer gave the most universal and highest enhancement of gene expression levels .
	manualset3
168113	4	412886	7	NULL	NULL	0	NULL	highest enhancement	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The tripartite leader sequence of human adenovirus mRNA linked with a major late promoter enhancer gave the most universal and highest enhancement of gene expression levels .
	manualset3
168114	5	412886	7	NULL	NULL	0	NULL	gene expression levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The tripartite leader sequence of human adenovirus mRNA linked with a major late promoter enhancer gave the most universal and highest enhancement of gene expression levels .
	manualset3
168115	1	412887	7	NULL	NULL	0	NULL	true digestible amino acid contents	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The true digestible amino acid contents in the basal diet were determined using the precision-fed assay with adult cecectomized roosters .
	manualset3
168116	2	412887	7	NULL	NULL	0	NULL	basal diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The true digestible amino acid contents in the basal diet were determined using the precision-fed assay with adult cecectomized roosters .
	manualset3
168117	3	412887	7	NULL	NULL	0	NULL	precision-fed assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The true digestible amino acid contents in the basal diet were determined using the precision-fed assay with adult cecectomized roosters .
	manualset3
168118	4	412887	7	NULL	NULL	0	NULL	adult cecectomized roosters	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The true digestible amino acid contents in the basal diet were determined using the precision-fed assay with adult cecectomized roosters .
	manualset3
168119	1	412888	7	NULL	NULL	0	NULL	 truncation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The truncation probably impairs the TrpA activity , thus elucidating a possible molecular mechanism behind variations in the pathogenesis of C. trachomatis serovars .
	manualset3
168120	2	412888	7	NULL	NULL	0	NULL	TrpA activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The truncation probably impairs the TrpA activity , thus elucidating a possible molecular mechanism behind variations in the pathogenesis of C. trachomatis serovars .
	manualset3
168121	3	412888	7	NULL	NULL	0	NULL	molecular mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The truncation probably impairs the TrpA activity , thus elucidating a possible molecular mechanism behind variations in the pathogenesis of C. trachomatis serovars .
	manualset3
168122	4	412888	7	NULL	NULL	0	NULL	variations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The truncation probably impairs the TrpA activity , thus elucidating a possible molecular mechanism behind variations in the pathogenesis of C. trachomatis serovars .
	manualset3
168123	5	412888	7	NULL	NULL	0	NULL	pathogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The truncation probably impairs the TrpA activity , thus elucidating a possible molecular mechanism behind variations in the pathogenesis of C. trachomatis serovars .
	manualset3
168124	6	412888	7	NULL	NULL	0	NULL	C. trachomatis serovars	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The truncation probably impairs the TrpA activity , thus elucidating a possible molecular mechanism behind variations in the pathogenesis of C. trachomatis serovars .
	manualset3
168126	1	412889	7	NULL	NULL	0	NULL	tuberculosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The tuberculosis or HIV-infected patients were more frequently found to have Chylomastix mesnili , Jodamoeba butschlii , and Endolimax nana .
	manualset3
168127	2	412889	7	NULL	NULL	0	NULL	HIV-infected patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The tuberculosis or HIV-infected patients were more frequently found to have Chylomastix mesnili , Jodamoeba butschlii , and Endolimax nana .
	manualset3
168128	3	412889	7	NULL	NULL	0	NULL	Chylomastix mesnili 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The tuberculosis or HIV-infected patients were more frequently found to have Chylomastix mesnili , Jodamoeba butschlii , and Endolimax nana .
	manualset3
168129	4	412889	7	NULL	NULL	0	NULL	Jodamoeba butschlii 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The tuberculosis or HIV-infected patients were more frequently found to have Chylomastix mesnili , Jodamoeba butschlii , and Endolimax nana .
	manualset3
168130	5	412889	7	NULL	NULL	0	NULL	Endolimax nana	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The tuberculosis or HIV-infected patients were more frequently found to have Chylomastix mesnili , Jodamoeba butschlii , and Endolimax nana .
	manualset3
168131	1	412890	7	NULL	NULL	0	NULL	tumor-suppressive property	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The tumor-suppressive property of hCG against palpable N-methyl-N-nitrosourea ( MNU ) - induced rat mammary carcinomas was examined .
	manualset3
168132	2	412890	7	NULL	NULL	0	NULL	 hCG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The tumor-suppressive property of hCG against palpable N-methyl-N-nitrosourea ( MNU ) - induced rat mammary carcinomas was examined .
	manualset3
168133	3	412890	7	NULL	NULL	0	NULL	 palpable N-methyl-N-nitrosourea ( MNU ) - induced rat mammary carcinomas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The tumor-suppressive property of hCG against palpable N-methyl-N-nitrosourea ( MNU ) - induced rat mammary carcinomas was examined .
	manualset3
168134	1	412891	7	NULL	NULL	0	NULL	tumor 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The tumor is most often localized in the femur ; it is not unusual to find it in the tibia , maxilla and mandible .
	manualset3
168135	2	412891	7	NULL	NULL	0	NULL	femur	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The tumor is most often localized in the femur ; it is not unusual to find it in the tibia , maxilla and mandible .
	manualset3
168136	3	412891	7	NULL	NULL	0	NULL	tibia	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The tumor is most often localized in the femur ; it is not unusual to find it in the tibia , maxilla and mandible .
	manualset3
168137	4	412891	7	NULL	NULL	0	NULL	maxilla 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The tumor is most often localized in the femur ; it is not unusual to find it in the tibia , maxilla and mandible .
	manualset3
168138	5	412891	7	NULL	NULL	0	NULL	mandible	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The tumor is most often localized in the femur ; it is not unusual to find it in the tibia , maxilla and mandible .
	manualset3
168139	1	412892	7	NULL	NULL	0	NULL	tumor margins	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The tumor margins were marked on the basis of FD .
	manualset3
168140	2	412892	7	NULL	NULL	0	NULL	 basis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The tumor margins were marked on the basis of FD .
	manualset3
168141	3	412892	7	NULL	NULL	0	NULL	FD	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The tumor margins were marked on the basis of FD .
	manualset3
168142	1	412893	7	NULL	NULL	0	NULL	 tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The tumor was evaluated by light microscopy , immunocytochemistry , electron microscopy , cytogenetics , and molecular genetics .
	manualset3
168143	2	412893	7	NULL	NULL	NULL	NULL	light microscopy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The tumor was evaluated by light microscopy , immunocytochemistry , electron microscopy , cytogenetics , and molecular genetics .
	manualset3
168144	3	412893	7	NULL	NULL	NULL	NULL	immunocytochemistry	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The tumor was evaluated by light microscopy , immunocytochemistry , electron microscopy , cytogenetics , and molecular genetics .
	manualset3
168145	4	412893	7	NULL	NULL	NULL	NULL	electron microscopy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The tumor was evaluated by light microscopy , immunocytochemistry , electron microscopy , cytogenetics , and molecular genetics .
	manualset3
168146	5	412893	7	NULL	NULL	NULL	NULL	cytogenetics	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The tumor was evaluated by light microscopy , immunocytochemistry , electron microscopy , cytogenetics , and molecular genetics .
	manualset3
168147	6	412893	7	NULL	NULL	NULL	NULL	molecular genetics	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The tumor was evaluated by light microscopy , immunocytochemistry , electron microscopy , cytogenetics , and molecular genetics .
	manualset3
168148	1	412894	7	NULL	NULL	0	NULL	 tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The tumor was totally resected via a parietal , transventricular approach .
	manualset3
168149	2	412894	7	NULL	NULL	0	NULL	parietal , transventricular approach	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The tumor was totally resected via a parietal , transventricular approach .
	manualset3
168150	1	412895	7	NULL	NULL	0	NULL	tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The tumors that developed following inoculation of hybrid cells into BALB/c mice ( 1 x 10 ( 6 ) cells/mouse ) were karyotypically identical to the inoculated cells .
	manualset3
168151	2	412895	7	NULL	NULL	0	NULL	inoculation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The tumors that developed following inoculation of hybrid cells into BALB/c mice ( 1 x 10 ( 6 ) cells/mouse ) were karyotypically identical to the inoculated cells .
	manualset3
168152	3	412895	7	NULL	NULL	0	NULL	hybrid cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The tumors that developed following inoculation of hybrid cells into BALB/c mice ( 1 x 10 ( 6 ) cells/mouse ) were karyotypically identical to the inoculated cells .
	manualset3
168153	4	412895	7	NULL	NULL	0	NULL	BALB/c mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The tumors that developed following inoculation of hybrid cells into BALB/c mice ( 1 x 10 ( 6 ) cells/mouse ) were karyotypically identical to the inoculated cells .
	manualset3
168154	5	412895	7	NULL	NULL	0	NULL	1 x 10 ( 6 ) cells/mouse	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The tumors that developed following inoculation of hybrid cells into BALB/c mice ( 1 x 10 ( 6 ) cells/mouse ) were karyotypically identical to the inoculated cells .
	manualset3
168155	6	412895	7	NULL	NULL	0	NULL	 inoculated cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The tumors that developed following inoculation of hybrid cells into BALB/c mice ( 1 x 10 ( 6 ) cells/mouse ) were karyotypically identical to the inoculated cells .
	manualset3
168156	1	412896	7	NULL	NULL	0	NULL	tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The tumors were compared histologically to 147 intraparenchymal hamartomas studied during the same period .
	manualset3
168157	2	412896	7	NULL	NULL	0	NULL	 147 intraparenchymal hamartomas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The tumors were compared histologically to 147 intraparenchymal hamartomas studied during the same period .
	manualset3
168158	3	412896	7	NULL	NULL	0	NULL	period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The tumors were compared histologically to 147 intraparenchymal hamartomas studied during the same period .
	manualset3
168159	1	412897	7	NULL	NULL	0	NULL	tunica media	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The tunica media of the cranial vena cava was composed of cardiac myocytes after formation of the endothelium .
	manualset3
168160	2	412897	7	NULL	NULL	0	NULL	cranial vena cava	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The tunica media of the cranial vena cava was composed of cardiac myocytes after formation of the endothelium .
	manualset3
168161	3	412897	7	NULL	NULL	0	NULL	cardiac myocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The tunica media of the cranial vena cava was composed of cardiac myocytes after formation of the endothelium .
	manualset3
168162	4	412897	7	NULL	NULL	0	NULL	formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The tunica media of the cranial vena cava was composed of cardiac myocytes after formation of the endothelium .
	manualset3
168163	5	412897	7	NULL	NULL	0	NULL	endothelium 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The tunica media of the cranial vena cava was composed of cardiac myocytes after formation of the endothelium .
	manualset3
168164	1	412898	7	NULL	NULL	0	NULL	turbulence dissipation coefficient	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The turbulence dissipation coefficient decreases very slightlywith increasing solids fraction for both systems .
	manualset3
168165	2	412898	7	NULL	NULL	0	NULL	increasing solids fraction	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The turbulence dissipation coefficient decreases very slightlywith increasing solids fraction for both systems .
	manualset3
168166	3	412898	7	NULL	NULL	0	NULL	systems 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The turbulence dissipation coefficient decreases very slightlywith increasing solids fraction for both systems .
	manualset3
168167	1	412899	7	NULL	NULL	0	NULL	turnover number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The turnover number of the purified enzyme dimer is approx .
	manualset3
168168	2	412899	7	NULL	NULL	0	NULL	purified enzyme dimer	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The turnover number of the purified enzyme dimer is approx .
	manualset3
168169	1	412900	7	NULL	NULL	0	NULL	turnover	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The turnover of 5-hydroxytryptamine in both the denervated and the reinnervated hippocampus was comparable to that in control tissue .
	manualset3
168170	2	412900	7	NULL	NULL	0	NULL	5-hydroxytryptamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The turnover of 5-hydroxytryptamine in both the denervated and the reinnervated hippocampus was comparable to that in control tissue .
	manualset3
168171	3	412900	7	NULL	NULL	0	NULL	denervated hippocampus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The turnover of 5-hydroxytryptamine in both the denervated and the reinnervated hippocampus was comparable to that in control tissue .
	manualset3
168172	4	412900	7	NULL	NULL	0	NULL	reinnervated hippocampus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The turnover of 5-hydroxytryptamine in both the denervated and the reinnervated hippocampus was comparable to that in control tissue .
	manualset3
168173	5	412900	7	NULL	NULL	0	NULL	control tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The turnover of 5-hydroxytryptamine in both the denervated and the reinnervated hippocampus was comparable to that in control tissue .
	manualset3
168174	1	412901	7	NULL	NULL	0	NULL	Acromegaly	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acromegaly and hyperprolactinemia in McCune-Albright syndrome .
	manualset3
168175	2	412901	7	NULL	NULL	0	NULL	hyperprolactinemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acromegaly and hyperprolactinemia in McCune-Albright syndrome .
	manualset3
168176	3	412901	7	NULL	NULL	0	NULL	McCune-Albright syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Acromegaly and hyperprolactinemia in McCune-Albright syndrome .
	manualset3
168177	1	412902	7	NULL	NULL	0	NULL	two-repeat fragment ( B1B2 )	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The two-repeat fragment ( B1B2 ) crystallized in the orthorhombic space group P212121 with cell dimensions a = 42.4 , b = 79.4 , c = 130.4 A and diffracted to 2.3 A resolution .
	manualset3
168178	2	412902	7	NULL	NULL	0	NULL	 orthorhombic space group P212121	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The two-repeat fragment ( B1B2 ) crystallized in the orthorhombic space group P212121 with cell dimensions a = 42.4 , b = 79.4 , c = 130.4 A and diffracted to 2.3 A resolution .
	manualset3
168179	3	412902	7	NULL	NULL	0	NULL	cell dimensions	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The two-repeat fragment ( B1B2 ) crystallized in the orthorhombic space group P212121 with cell dimensions a = 42.4 , b = 79.4 , c = 130.4 A and diffracted to 2.3 A resolution .
	manualset3
168180	4	412902	7	NULL	NULL	0	NULL	a = 42.4 , b = 79.4 , c = 130.4 A	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The two-repeat fragment ( B1B2 ) crystallized in the orthorhombic space group P212121 with cell dimensions a = 42.4 , b = 79.4 , c = 130.4 A and diffracted to 2.3 A resolution .
	manualset3
168181	5	412902	7	NULL	NULL	0	NULL	2.3 A resolution	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The two-repeat fragment ( B1B2 ) crystallized in the orthorhombic space group P212121 with cell dimensions a = 42.4 , b = 79.4 , c = 130.4 A and diffracted to 2.3 A resolution .
	manualset3
168182	1	412903	7	NULL	NULL	0	NULL	two-step self-etch adhesive	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The two-step self-etch adhesive was not influenced by selective enamel etching or by the LED-curing unit .
	manualset3
168183	2	412903	7	NULL	NULL	0	NULL	selective enamel etching	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The two-step self-etch adhesive was not influenced by selective enamel etching or by the LED-curing unit .
	manualset3
168184	3	412903	7	NULL	NULL	NULL	NULL	LED-curing unit	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The two-step self-etch adhesive was not influenced by selective enamel etching or by the LED-curing unit .
	manualset3
168185	1	412904	7	NULL	NULL	0	NULL	two - SH groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The two - SH groups of S1 are located in the central region of the chain at positions 292 and 349 , the latter being the reactive group whose modification results in the reported loss of the nucleic-acid-unfolding ability of S1 .
	manualset3
168186	2	412904	7	NULL	NULL	NULL	NULL	S1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The two - SH groups of S1 are located in the central region of the chain at positions 292 and 349 , the latter being the reactive group whose modification results in the reported loss of the nucleic-acid-unfolding ability of S1 .
	manualset3
168187	3	412904	7	NULL	NULL	0	NULL	central region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The two - SH groups of S1 are located in the central region of the chain at positions 292 and 349 , the latter being the reactive group whose modification results in the reported loss of the nucleic-acid-unfolding ability of S1 .
	manualset3
168188	4	412904	7	NULL	NULL	0	NULL	chain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The two - SH groups of S1 are located in the central region of the chain at positions 292 and 349 , the latter being the reactive group whose modification results in the reported loss of the nucleic-acid-unfolding ability of S1 .
	manualset3
168189	5	412904	7	NULL	NULL	NULL	NULL	positions 292	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The two - SH groups of S1 are located in the central region of the chain at positions 292 and 349 , the latter being the reactive group whose modification results in the reported loss of the nucleic-acid-unfolding ability of S1 .
	manualset3
168190	6	412904	7	NULL	NULL	0	NULL	positions 349	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The two - SH groups of S1 are located in the central region of the chain at positions 292 and 349 , the latter being the reactive group whose modification results in the reported loss of the nucleic-acid-unfolding ability of S1 .
	manualset3
168191	7	412904	7	NULL	NULL	0	NULL	reactive group	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The two - SH groups of S1 are located in the central region of the chain at positions 292 and 349 , the latter being the reactive group whose modification results in the reported loss of the nucleic-acid-unfolding ability of S1 .
	manualset3
168192	8	412904	7	NULL	NULL	0	NULL	modification	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The two - SH groups of S1 are located in the central region of the chain at positions 292 and 349 , the latter being the reactive group whose modification results in the reported loss of the nucleic-acid-unfolding ability of S1 .
	manualset3
168193	9	412904	7	NULL	NULL	0	NULL	reported loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The two - SH groups of S1 are located in the central region of the chain at positions 292 and 349 , the latter being the reactive group whose modification results in the reported loss of the nucleic-acid-unfolding ability of S1 .
	manualset3
168194	10	412904	7	NULL	NULL	0	NULL	nucleic-acid-unfolding ability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The two - SH groups of S1 are located in the central region of the chain at positions 292 and 349 , the latter being the reactive group whose modification results in the reported loss of the nucleic-acid-unfolding ability of S1 .
	manualset3
168195	11	412904	7	NULL	NULL	0	NULL	 S1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The two - SH groups of S1 are located in the central region of the chain at positions 292 and 349 , the latter being the reactive group whose modification results in the reported loss of the nucleic-acid-unfolding ability of S1 .
	manualset3
168196	1	412905	7	NULL	NULL	0	NULL	 two central helices	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The two central helices and a connecting loop in large T antigen have structural similarities with the J domains of the molecular chaperones DnaJ and HDJ-1 , suggesting that large T antigen may use a chaperone mechanism for its biological function .
	manualset3
168197	2	412905	7	NULL	NULL	0	NULL	connecting loop	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The two central helices and a connecting loop in large T antigen have structural similarities with the J domains of the molecular chaperones DnaJ and HDJ-1 , suggesting that large T antigen may use a chaperone mechanism for its biological function .
	manualset3
168198	3	412905	7	NULL	NULL	0	NULL	large T antigen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The two central helices and a connecting loop in large T antigen have structural similarities with the J domains of the molecular chaperones DnaJ and HDJ-1 , suggesting that large T antigen may use a chaperone mechanism for its biological function .
	manualset3
168199	4	412905	7	NULL	NULL	0	NULL	structural similarities	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The two central helices and a connecting loop in large T antigen have structural similarities with the J domains of the molecular chaperones DnaJ and HDJ-1 , suggesting that large T antigen may use a chaperone mechanism for its biological function .
	manualset3
168200	5	412905	7	NULL	NULL	0	NULL	J domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The two central helices and a connecting loop in large T antigen have structural similarities with the J domains of the molecular chaperones DnaJ and HDJ-1 , suggesting that large T antigen may use a chaperone mechanism for its biological function .
	manualset3
168201	6	412905	7	NULL	NULL	0	NULL	molecular chaperones	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The two central helices and a connecting loop in large T antigen have structural similarities with the J domains of the molecular chaperones DnaJ and HDJ-1 , suggesting that large T antigen may use a chaperone mechanism for its biological function .
	manualset3
168202	7	412905	7	NULL	NULL	0	NULL	DnaJ	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The two central helices and a connecting loop in large T antigen have structural similarities with the J domains of the molecular chaperones DnaJ and HDJ-1 , suggesting that large T antigen may use a chaperone mechanism for its biological function .
	manualset3
168203	8	412905	7	NULL	NULL	0	NULL	HDJ-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The two central helices and a connecting loop in large T antigen have structural similarities with the J domains of the molecular chaperones DnaJ and HDJ-1 , suggesting that large T antigen may use a chaperone mechanism for its biological function .
	manualset3
168204	9	412905	7	NULL	NULL	0	NULL	large T antigen 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The two central helices and a connecting loop in large T antigen have structural similarities with the J domains of the molecular chaperones DnaJ and HDJ-1 , suggesting that large T antigen may use a chaperone mechanism for its biological function .
	manualset3
168205	10	412905	7	NULL	NULL	0	NULL	chaperone mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The two central helices and a connecting loop in large T antigen have structural similarities with the J domains of the molecular chaperones DnaJ and HDJ-1 , suggesting that large T antigen may use a chaperone mechanism for its biological function .
	manualset3
168206	11	412905	7	NULL	NULL	0	NULL	 biological function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The two central helices and a connecting loop in large T antigen have structural similarities with the J domains of the molecular chaperones DnaJ and HDJ-1 , suggesting that large T antigen may use a chaperone mechanism for its biological function .
	manualset3
168207	1	412906	7	NULL	NULL	NULL	NULL	two drug groups	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The two drug groups delivered litters significantly later with evidence of increased resorption at the higher dose .
	manualset3
168208	2	412906	7	NULL	NULL	NULL	NULL	evidence 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The two drug groups delivered litters significantly later with evidence of increased resorption at the higher dose .
	manualset3
168209	3	412906	7	NULL	NULL	0	NULL	increased resorption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The two drug groups delivered litters significantly later with evidence of increased resorption at the higher dose .
	manualset3
168210	4	412906	7	NULL	NULL	0	NULL	higher dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The two drug groups delivered litters significantly later with evidence of increased resorption at the higher dose .
	manualset3
169720	5	412906	7	NULL	NULL	0	NULL	litters	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The two drug groups delivered litters significantly later with evidence of increased resorption at the higher dose .
	manualset3
168211	1	412907	7	NULL	NULL	0	NULL	 two forms	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The two forms of alpha-galactosidases A and B used in this study were extensively purified by classical procedures .
	manualset3
168212	2	412907	7	NULL	NULL	0	NULL	alpha-galactosidases A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The two forms of alpha-galactosidases A and B used in this study were extensively purified by classical procedures .
	manualset3
168213	3	412907	7	NULL	NULL	0	NULL	alpha-galactosidases B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The two forms of alpha-galactosidases A and B used in this study were extensively purified by classical procedures .
	manualset3
168214	4	412907	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The two forms of alpha-galactosidases A and B used in this study were extensively purified by classical procedures .
	manualset3
168215	5	412907	7	NULL	NULL	0	NULL	classical procedures	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The two forms of alpha-galactosidases A and B used in this study were extensively purified by classical procedures .
	manualset3
168216	1	412908	7	NULL	NULL	0	NULL	two human 3 beta-HSD genes 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The two human 3 beta-HSD genes and the three related pseudogenes are located on the chromosome 1p13 .1 region , close to the centromeric marker D1Z5 .
	manualset3
168217	2	412908	7	NULL	NULL	0	NULL	three related pseudogenes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The two human 3 beta-HSD genes and the three related pseudogenes are located on the chromosome 1p13 .1 region , close to the centromeric marker D1Z5 .
	manualset3
168218	3	412908	7	NULL	NULL	0	NULL	chromosome 1p13 .1 region	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The two human 3 beta-HSD genes and the three related pseudogenes are located on the chromosome 1p13 .1 region , close to the centromeric marker D1Z5 .
	manualset3
168219	4	412908	7	NULL	NULL	NULL	NULL	centromeric marker D1Z5	Chromosome												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The two human 3 beta-HSD genes and the three related pseudogenes are located on the chromosome 1p13 .1 region , close to the centromeric marker D1Z5 .
	manualset3
168220	1	412909	7	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The two initial 3-phosphoglycerate substrate molecules near the active centers of the initial structure of PGM have been replaced with final product ( 2-phosphoglycerate ) molecules , and 150 mM NaCl together with three Mg2 + ions have been added to the system to observe post-catalytic activity under near-physiological conditions .
	manualset3
168221	2	412909	7	NULL	NULL	0	NULL	3-phosphoglycerate substrate molecules	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The two initial 3-phosphoglycerate substrate molecules near the active centers of the initial structure of PGM have been replaced with final product ( 2-phosphoglycerate ) molecules , and 150 mM NaCl together with three Mg2 + ions have been added to the system to observe post-catalytic activity under near-physiological conditions .
	manualset3
168222	3	412909	7	NULL	NULL	0	NULL	active centers	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The two initial 3-phosphoglycerate substrate molecules near the active centers of the initial structure of PGM have been replaced with final product ( 2-phosphoglycerate ) molecules , and 150 mM NaCl together with three Mg2 + ions have been added to the system to observe post-catalytic activity under near-physiological conditions .
	manualset3
168223	4	412909	7	NULL	NULL	0	NULL	initial structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The two initial 3-phosphoglycerate substrate molecules near the active centers of the initial structure of PGM have been replaced with final product ( 2-phosphoglycerate ) molecules , and 150 mM NaCl together with three Mg2 + ions have been added to the system to observe post-catalytic activity under near-physiological conditions .
	manualset3
168224	5	412909	7	NULL	NULL	0	NULL	PGM	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The two initial 3-phosphoglycerate substrate molecules near the active centers of the initial structure of PGM have been replaced with final product ( 2-phosphoglycerate ) molecules , and 150 mM NaCl together with three Mg2 + ions have been added to the system to observe post-catalytic activity under near-physiological conditions .
	manualset3
168225	6	412909	7	NULL	NULL	0	NULL	final product	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The two initial 3-phosphoglycerate substrate molecules near the active centers of the initial structure of PGM have been replaced with final product ( 2-phosphoglycerate ) molecules , and 150 mM NaCl together with three Mg2 + ions have been added to the system to observe post-catalytic activity under near-physiological conditions .
	manualset3
168226	7	412909	7	NULL	NULL	0	NULL	(2-phosphoglycerate ) molecules	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The two initial 3-phosphoglycerate substrate molecules near the active centers of the initial structure of PGM have been replaced with final product ( 2-phosphoglycerate ) molecules , and 150 mM NaCl together with three Mg2 + ions have been added to the system to observe post-catalytic activity under near-physiological conditions .
	manualset3
168227	8	412909	7	NULL	NULL	0	NULL	150 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The two initial 3-phosphoglycerate substrate molecules near the active centers of the initial structure of PGM have been replaced with final product ( 2-phosphoglycerate ) molecules , and 150 mM NaCl together with three Mg2 + ions have been added to the system to observe post-catalytic activity under near-physiological conditions .
	manualset3
168228	9	412909	7	NULL	NULL	0	NULL	NaCl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The two initial 3-phosphoglycerate substrate molecules near the active centers of the initial structure of PGM have been replaced with final product ( 2-phosphoglycerate ) molecules , and 150 mM NaCl together with three Mg2 + ions have been added to the system to observe post-catalytic activity under near-physiological conditions .
	manualset3
168229	10	412909	7	NULL	NULL	0	NULL	three Mg2 + ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The two initial 3-phosphoglycerate substrate molecules near the active centers of the initial structure of PGM have been replaced with final product ( 2-phosphoglycerate ) molecules , and 150 mM NaCl together with three Mg2 + ions have been added to the system to observe post-catalytic activity under near-physiological conditions .
	manualset3
168230	11	412909	7	NULL	NULL	0	NULL	system	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The two initial 3-phosphoglycerate substrate molecules near the active centers of the initial structure of PGM have been replaced with final product ( 2-phosphoglycerate ) molecules , and 150 mM NaCl together with three Mg2 + ions have been added to the system to observe post-catalytic activity under near-physiological conditions .
	manualset3
168231	12	412909	7	NULL	NULL	0	NULL	post-catalytic activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The two initial 3-phosphoglycerate substrate molecules near the active centers of the initial structure of PGM have been replaced with final product ( 2-phosphoglycerate ) molecules , and 150 mM NaCl together with three Mg2 + ions have been added to the system to observe post-catalytic activity under near-physiological conditions .
	manualset3
168232	13	412909	7	NULL	NULL	0	NULL	near-physiological conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The two initial 3-phosphoglycerate substrate molecules near the active centers of the initial structure of PGM have been replaced with final product ( 2-phosphoglycerate ) molecules , and 150 mM NaCl together with three Mg2 + ions have been added to the system to observe post-catalytic activity under near-physiological conditions .
	manualset3
168233	1	412910	7	NULL	NULL	0	NULL	Canada	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Across Canada , experience with screening for distress is growing , as cancer facilities implement screening programs .
	manualset3
168234	2	412910	7	NULL	NULL	0	NULL	screening	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Across Canada , experience with screening for distress is growing , as cancer facilities implement screening programs .
	manualset3
168235	3	412910	7	NULL	NULL	0	NULL	distress 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Across Canada , experience with screening for distress is growing , as cancer facilities implement screening programs .
	manualset3
168237	5	412910	7	NULL	NULL	0	NULL	cancer facilities	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Across Canada , experience with screening for distress is growing , as cancer facilities implement screening programs .
	manualset3
168238	6	412910	7	NULL	NULL	0	NULL	screening programs	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Across Canada , experience with screening for distress is growing , as cancer facilities implement screening programs .
	manualset3
168239	7	412910	7	NULL	NULL	0	NULL	experience	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Across Canada , experience with screening for distress is growing , as cancer facilities implement screening programs .
	manualset3
168240	1	412911	7	NULL	NULL	0	NULL	two title chromene compounds 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The two title chromene compounds , 3 , 3a-dihydrocyclopenta ( b ) chromen-1 ( 2H ) - one , C16H12O2 , ( I ) , and 2 - ( 2-hydroxybenzylidene ) -3 , 3 a-dihydrocyclopenta ( b ) chromen-1 ( 2H ) - one , C19H14O3 , ( II ) , have been determined in the monoclinic space group P2 ( 1 ) / n. Compound ( I ) is mainly stabilized by C-H ... pi interactions .
	manualset3
168241	2	412911	7	NULL	NULL	0	NULL	3 , 3a-dihydrocyclopenta ( b ) chromen-1 ( 2H ) - one	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The two title chromene compounds , 3 , 3a-dihydrocyclopenta ( b ) chromen-1 ( 2H ) - one , C16H12O2 , ( I ) , and 2 - ( 2-hydroxybenzylidene ) -3 , 3 a-dihydrocyclopenta ( b ) chromen-1 ( 2H ) - one , C19H14O3 , ( II ) , have been determined in the monoclinic space group P2 ( 1 ) / n. Compound ( I ) is mainly stabilized by C-H ... pi interactions .
	manualset3
168242	3	412911	7	NULL	NULL	0	NULL	C16H12O2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The two title chromene compounds , 3 , 3a-dihydrocyclopenta ( b ) chromen-1 ( 2H ) - one , C16H12O2 , ( I ) , and 2 - ( 2-hydroxybenzylidene ) -3 , 3 a-dihydrocyclopenta ( b ) chromen-1 ( 2H ) - one , C19H14O3 , ( II ) , have been determined in the monoclinic space group P2 ( 1 ) / n. Compound ( I ) is mainly stabilized by C-H ... pi interactions .
	manualset3
168243	4	412911	7	NULL	NULL	0	NULL	2 - ( 2-hydroxybenzylidene ) -3 , 3 a-dihydrocyclopenta ( b ) chromen-1 ( 2H ) - one	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The two title chromene compounds , 3 , 3a-dihydrocyclopenta ( b ) chromen-1 ( 2H ) - one , C16H12O2 , ( I ) , and 2 - ( 2-hydroxybenzylidene ) -3 , 3 a-dihydrocyclopenta ( b ) chromen-1 ( 2H ) - one , C19H14O3 , ( II ) , have been determined in the monoclinic space group P2 ( 1 ) / n. Compound ( I ) is mainly stabilized by C-H ... pi interactions .
	manualset3
168244	5	412911	7	NULL	NULL	NULL	NULL	C19H14O3 , ( II ) ,	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The two title chromene compounds , 3 , 3a-dihydrocyclopenta ( b ) chromen-1 ( 2H ) - one , C16H12O2 , ( I ) , and 2 - ( 2-hydroxybenzylidene ) -3 , 3 a-dihydrocyclopenta ( b ) chromen-1 ( 2H ) - one , C19H14O3 , ( II ) , have been determined in the monoclinic space group P2 ( 1 ) / n. Compound ( I ) is mainly stabilized by C-H ... pi interactions .
	manualset3
168245	6	412911	7	NULL	NULL	0	NULL	monoclinic space group P2 ( 1 ) / n	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The two title chromene compounds , 3 , 3a-dihydrocyclopenta ( b ) chromen-1 ( 2H ) - one , C16H12O2 , ( I ) , and 2 - ( 2-hydroxybenzylidene ) -3 , 3 a-dihydrocyclopenta ( b ) chromen-1 ( 2H ) - one , C19H14O3 , ( II ) , have been determined in the monoclinic space group P2 ( 1 ) / n. Compound ( I ) is mainly stabilized by C-H ... pi interactions .
	manualset3
168246	7	412911	7	NULL	NULL	0	NULL	Compound ( I )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The two title chromene compounds , 3 , 3a-dihydrocyclopenta ( b ) chromen-1 ( 2H ) - one , C16H12O2 , ( I ) , and 2 - ( 2-hydroxybenzylidene ) -3 , 3 a-dihydrocyclopenta ( b ) chromen-1 ( 2H ) - one , C19H14O3 , ( II ) , have been determined in the monoclinic space group P2 ( 1 ) / n. Compound ( I ) is mainly stabilized by C-H ... pi interactions .
	manualset3
168247	8	412911	7	NULL	NULL	0	NULL	C-H ... pi interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The two title chromene compounds , 3 , 3a-dihydrocyclopenta ( b ) chromen-1 ( 2H ) - one , C16H12O2 , ( I ) , and 2 - ( 2-hydroxybenzylidene ) -3 , 3 a-dihydrocyclopenta ( b ) chromen-1 ( 2H ) - one , C19H14O3 , ( II ) , have been determined in the monoclinic space group P2 ( 1 ) / n. Compound ( I ) is mainly stabilized by C-H ... pi interactions .
	manualset3
168248	1	412912	7	NULL	NULL	0	NULL	two treatments	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The two treatments did not differ from each other on any of the outcome variables .
	manualset3
168249	2	412912	7	NULL	NULL	0	NULL	outcome variables	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The two treatments did not differ from each other on any of the outcome variables .
	manualset3
168250	1	412913	7	NULL	NULL	0	NULL	 type 1 insulin-like growth factor receptor ( IGF-1R )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The type 1 insulin-like growth factor receptor ( IGF-1R ) , a transmembrane tyrosine kinase , is widely expressed across many cell types in foetal and postnatal tissues .
	manualset3
168251	2	412913	7	NULL	NULL	0	NULL	transmembrane tyrosine kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The type 1 insulin-like growth factor receptor ( IGF-1R ) , a transmembrane tyrosine kinase , is widely expressed across many cell types in foetal and postnatal tissues .
	manualset3
168252	3	412913	7	NULL	NULL	0	NULL	cell types	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The type 1 insulin-like growth factor receptor ( IGF-1R ) , a transmembrane tyrosine kinase , is widely expressed across many cell types in foetal and postnatal tissues .
	manualset3
168253	4	412913	7	NULL	NULL	0	NULL	foetal tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The type 1 insulin-like growth factor receptor ( IGF-1R ) , a transmembrane tyrosine kinase , is widely expressed across many cell types in foetal and postnatal tissues .
	manualset3
168254	5	412913	7	NULL	NULL	0	NULL	postnatal tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The type 1 insulin-like growth factor receptor ( IGF-1R ) , a transmembrane tyrosine kinase , is widely expressed across many cell types in foetal and postnatal tissues .
	manualset3
168255	1	412914	7	NULL	NULL	0	NULL	type	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The type of school attended is used as a measure for outcome of preschool intervention .
	manualset3
168256	2	412914	7	NULL	NULL	0	NULL	 school	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The type of school attended is used as a measure for outcome of preschool intervention .
	manualset3
168257	3	412914	7	NULL	NULL	0	NULL	 measure 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The type of school attended is used as a measure for outcome of preschool intervention .
	manualset3
168258	4	412914	7	NULL	NULL	0	NULL	outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The type of school attended is used as a measure for outcome of preschool intervention .
	manualset3
168259	5	412914	7	NULL	NULL	0	NULL	 preschool intervention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The type of school attended is used as a measure for outcome of preschool intervention .
	manualset3
168260	1	412915	7	NULL	NULL	0	NULL	Acrylamide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Acrylamide disrupts elemental composition and water content of rat tibial nerve .
	manualset3
168261	2	412915	7	NULL	NULL	0	NULL	elemental composition 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Acrylamide disrupts elemental composition and water content of rat tibial nerve .
	manualset3
168262	3	412915	7	NULL	NULL	0	NULL	water content	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Acrylamide disrupts elemental composition and water content of rat tibial nerve .
	manualset3
168263	4	412915	7	NULL	NULL	0	NULL	rat tibial nerve	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Acrylamide disrupts elemental composition and water content of rat tibial nerve .
	manualset3
168264	1	412916	7	NULL	NULL	0	NULL	types	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The types of IVSD included perimembrane ( 854 ) , outflow tract ( 131 ) and muscular ( 15 ) .
	manualset3
168265	2	412916	7	NULL	NULL	0	NULL	IVSD	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The types of IVSD included perimembrane ( 854 ) , outflow tract ( 131 ) and muscular ( 15 ) .
	manualset3
168266	3	412916	7	NULL	NULL	NULL	NULL	perimembrane ( 854 )	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The types of IVSD included perimembrane ( 854 ) , outflow tract ( 131 ) and muscular ( 15 ) .
	manualset3
168268	4	412916	7	NULL	NULL	NULL	NULL	outflow tract ( 131 )	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The types of IVSD included perimembrane ( 854 ) , outflow tract ( 131 ) and muscular ( 15 ) .
	manualset3
168270	5	412916	7	NULL	NULL	NULL	NULL	 muscular ( 15 )	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The types of IVSD included perimembrane ( 854 ) , outflow tract ( 131 ) and muscular ( 15 ) .
	manualset3
168272	1	412917	7	NULL	NULL	0	NULL	types	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The types of involvement that are most common are subarachnoid cysts which appear as intradural extramedullary masses and meningeal reaction with appearance of arachnoiditis at myelography .
	manualset3
168273	2	412917	7	NULL	NULL	0	NULL	involvement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The types of involvement that are most common are subarachnoid cysts which appear as intradural extramedullary masses and meningeal reaction with appearance of arachnoiditis at myelography .
	manualset3
168274	3	412917	7	NULL	NULL	0	NULL	subarachnoid cysts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The types of involvement that are most common are subarachnoid cysts which appear as intradural extramedullary masses and meningeal reaction with appearance of arachnoiditis at myelography .
	manualset3
168275	4	412917	7	NULL	NULL	0	NULL	intradural extramedullary masses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The types of involvement that are most common are subarachnoid cysts which appear as intradural extramedullary masses and meningeal reaction with appearance of arachnoiditis at myelography .
	manualset3
168276	5	412917	7	NULL	NULL	0	NULL	meningeal reaction 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The types of involvement that are most common are subarachnoid cysts which appear as intradural extramedullary masses and meningeal reaction with appearance of arachnoiditis at myelography .
	manualset3
168277	6	412917	7	NULL	NULL	0	NULL	appearance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The types of involvement that are most common are subarachnoid cysts which appear as intradural extramedullary masses and meningeal reaction with appearance of arachnoiditis at myelography .
	manualset3
168278	7	412917	7	NULL	NULL	0	NULL	arachnoiditis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The types of involvement that are most common are subarachnoid cysts which appear as intradural extramedullary masses and meningeal reaction with appearance of arachnoiditis at myelography .
	manualset3
168279	8	412917	7	NULL	NULL	0	NULL	myelography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The types of involvement that are most common are subarachnoid cysts which appear as intradural extramedullary masses and meningeal reaction with appearance of arachnoiditis at myelography .
	manualset3
168280	1	412918	7	NULL	NULL	0	NULL	tyrosine kinase EphrinA2 ( EphA2 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The tyrosine kinase EphrinA2 ( EphA2 ) , implicated in many cancers , was identified in this analysis .
	manualset3
168281	2	412918	7	NULL	NULL	NULL	NULL	cancers	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The tyrosine kinase EphrinA2 ( EphA2 ) , implicated in many cancers , was identified in this analysis .
	manualset3
168282	3	412918	7	NULL	NULL	0	NULL	 analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The tyrosine kinase EphrinA2 ( EphA2 ) , implicated in many cancers , was identified in this analysis .
	manualset3
168283	1	412919	7	NULL	NULL	0	NULL	 tyrosine kinase Pyk2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The tyrosine kinase Pyk2 was activated by tumor necrosis factor alpha , by ultraviolet irradiation , and by changes in osmolarity .
	manualset3
168284	2	412919	7	NULL	NULL	0	NULL	 tumor necrosis factor alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The tyrosine kinase Pyk2 was activated by tumor necrosis factor alpha , by ultraviolet irradiation , and by changes in osmolarity .
	manualset3
168285	3	412919	7	NULL	NULL	0	NULL	ultraviolet irradiation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The tyrosine kinase Pyk2 was activated by tumor necrosis factor alpha , by ultraviolet irradiation , and by changes in osmolarity .
	manualset3
168286	4	412919	7	NULL	NULL	0	NULL	changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The tyrosine kinase Pyk2 was activated by tumor necrosis factor alpha , by ultraviolet irradiation , and by changes in osmolarity .
	manualset3
168287	5	412919	7	NULL	NULL	0	NULL	osmolarity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The tyrosine kinase Pyk2 was activated by tumor necrosis factor alpha , by ultraviolet irradiation , and by changes in osmolarity .
	manualset3
168288	1	412920	7	NULL	NULL	0	NULL	ulcer	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The ulcer healed slowly , leaving a scar .
	manualset3
168289	2	412920	7	NULL	NULL	0	NULL	scar	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The ulcer healed slowly , leaving a scar .
	manualset3
168290	1	412921	7	NULL	NULL	0	NULL	ultrastructural finding	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ultrastructural finding revealed that the extent of cytopathology in the isthmus was greater than in the tubular shell gland and shell gland pouch .
	manualset3
168291	2	412921	7	NULL	NULL	0	NULL	extent of cytopathology 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The ultrastructural finding revealed that the extent of cytopathology in the isthmus was greater than in the tubular shell gland and shell gland pouch .
	manualset3
168292	3	412921	7	NULL	NULL	0	NULL	 isthmus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The ultrastructural finding revealed that the extent of cytopathology in the isthmus was greater than in the tubular shell gland and shell gland pouch .
	manualset3
168293	4	412921	7	NULL	NULL	0	NULL	tubular shell gland	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The ultrastructural finding revealed that the extent of cytopathology in the isthmus was greater than in the tubular shell gland and shell gland pouch .
	manualset3
168294	5	412921	7	NULL	NULL	0	NULL	shell gland pouch	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The ultrastructural finding revealed that the extent of cytopathology in the isthmus was greater than in the tubular shell gland and shell gland pouch .
	manualset3
168295	1	412922	7	NULL	NULL	0	NULL	ultrastructural identification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ultrastructural identification of reticulo-hypoglossal axon terminals anterogradely labeled with horseradish peroxidase .
	manualset3
168296	2	412922	7	NULL	NULL	0	NULL	reticulo-hypoglossal axon terminals	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The ultrastructural identification of reticulo-hypoglossal axon terminals anterogradely labeled with horseradish peroxidase .
	manualset3
168297	3	412922	7	NULL	NULL	0	NULL	horseradish peroxidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The ultrastructural identification of reticulo-hypoglossal axon terminals anterogradely labeled with horseradish peroxidase .
	manualset3
168298	1	412923	7	NULL	NULL	0	NULL	Acrylonitrile-butadiene-styrene ( ABS ) copolymers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Acrylonitrile-butadiene-styrene ( ABS ) copolymers without and with a polybrominated epoxy type flame retardant were thermally degraded at 450 degrees C alone ( 10 g ) and mixed with polyvinylchloride ( PVC ) ( 8 g/2 g ) .
	manualset3
168299	2	412923	7	NULL	NULL	0	NULL	polybrominated epoxy type flame retardant	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Acrylonitrile-butadiene-styrene ( ABS ) copolymers without and with a polybrominated epoxy type flame retardant were thermally degraded at 450 degrees C alone ( 10 g ) and mixed with polyvinylchloride ( PVC ) ( 8 g/2 g ) .
	manualset3
168300	3	412923	7	NULL	NULL	0	NULL	450 degrees C 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Acrylonitrile-butadiene-styrene ( ABS ) copolymers without and with a polybrominated epoxy type flame retardant were thermally degraded at 450 degrees C alone ( 10 g ) and mixed with polyvinylchloride ( PVC ) ( 8 g/2 g ) .
	manualset3
168301	4	412923	7	NULL	NULL	0	NULL	10 g	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Acrylonitrile-butadiene-styrene ( ABS ) copolymers without and with a polybrominated epoxy type flame retardant were thermally degraded at 450 degrees C alone ( 10 g ) and mixed with polyvinylchloride ( PVC ) ( 8 g/2 g ) .
	manualset3
168302	5	412923	7	NULL	NULL	0	NULL	polyvinylchloride ( PVC )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Acrylonitrile-butadiene-styrene ( ABS ) copolymers without and with a polybrominated epoxy type flame retardant were thermally degraded at 450 degrees C alone ( 10 g ) and mixed with polyvinylchloride ( PVC ) ( 8 g/2 g ) .
	manualset3
168303	6	412923	7	NULL	NULL	0	NULL	 8 g/2 g 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Acrylonitrile-butadiene-styrene ( ABS ) copolymers without and with a polybrominated epoxy type flame retardant were thermally degraded at 450 degrees C alone ( 10 g ) and mixed with polyvinylchloride ( PVC ) ( 8 g/2 g ) .
	manualset3
168304	1	412924	7	NULL	NULL	0	NULL	ultrastructure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ultrastructure of the DiC8-induced acrosomal loss was essentially identical to the acrosome reaction described for a broad range of placental mammals .
	manualset3
168305	2	412924	7	NULL	NULL	NULL	NULL	DiC8-induced acrosomal loss	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The ultrastructure of the DiC8-induced acrosomal loss was essentially identical to the acrosome reaction described for a broad range of placental mammals .
	manualset3
168306	3	412924	7	NULL	NULL	0	NULL	acrosome reaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ultrastructure of the DiC8-induced acrosomal loss was essentially identical to the acrosome reaction described for a broad range of placental mammals .
	manualset3
168307	4	412924	7	NULL	NULL	0	NULL	broad range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ultrastructure of the DiC8-induced acrosomal loss was essentially identical to the acrosome reaction described for a broad range of placental mammals .
	manualset3
168309	5	412924	7	NULL	NULL	0	NULL	placental mammals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The ultrastructure of the DiC8-induced acrosomal loss was essentially identical to the acrosome reaction described for a broad range of placental mammals .
	manualset3
169721	6	412924	7	NULL	NULL	0	NULL	identical	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The ultrastructure of the DiC8-induced acrosomal loss was essentially identical to the acrosome reaction described for a broad range of placental mammals .
	manualset3
168310	1	412925	7	NULL	NULL	0	NULL	ultrastructure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ultrastructure of the spines decorating the cladodes of the cactus Opuntia ficus-indica was investigated by optical microscopy , scanning and transmission electron microscopy , wide angle X-ray , and solid state 13C NMR analyses .
	manualset3
168311	2	412925	7	NULL	NULL	0	NULL	spines	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The ultrastructure of the spines decorating the cladodes of the cactus Opuntia ficus-indica was investigated by optical microscopy , scanning and transmission electron microscopy , wide angle X-ray , and solid state 13C NMR analyses .
	manualset3
168312	3	412925	7	NULL	NULL	0	NULL	cladodes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The ultrastructure of the spines decorating the cladodes of the cactus Opuntia ficus-indica was investigated by optical microscopy , scanning and transmission electron microscopy , wide angle X-ray , and solid state 13C NMR analyses .
	manualset3
168313	4	412925	7	NULL	NULL	0	NULL	 cactus Opuntia ficus-indica	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The ultrastructure of the spines decorating the cladodes of the cactus Opuntia ficus-indica was investigated by optical microscopy , scanning and transmission electron microscopy , wide angle X-ray , and solid state 13C NMR analyses .
	manualset3
168314	5	412925	7	NULL	NULL	0	NULL	optical microscopy 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ultrastructure of the spines decorating the cladodes of the cactus Opuntia ficus-indica was investigated by optical microscopy , scanning and transmission electron microscopy , wide angle X-ray , and solid state 13C NMR analyses .
	manualset3
168315	6	412925	7	NULL	NULL	0	NULL	scanning and transmission electron microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ultrastructure of the spines decorating the cladodes of the cactus Opuntia ficus-indica was investigated by optical microscopy , scanning and transmission electron microscopy , wide angle X-ray , and solid state 13C NMR analyses .
	manualset3
168316	7	412925	7	NULL	NULL	0	NULL	wide angle X-ray analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ultrastructure of the spines decorating the cladodes of the cactus Opuntia ficus-indica was investigated by optical microscopy , scanning and transmission electron microscopy , wide angle X-ray , and solid state 13C NMR analyses .
	manualset3
168317	8	412925	7	NULL	NULL	0	NULL	solid state 13C NMR analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ultrastructure of the spines decorating the cladodes of the cactus Opuntia ficus-indica was investigated by optical microscopy , scanning and transmission electron microscopy , wide angle X-ray , and solid state 13C NMR analyses .
	manualset3
168318	1	412926	7	NULL	NULL	0	NULL	unbinding of vortex defects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The unbinding of vortex defects in the superconducting condensate with d-wave symmetry at T = 0 is shown to lead to the insulator with incommensurate spin-density-wave order .
	manualset3
168319	2	412926	7	NULL	NULL	0	NULL	superconducting condensate	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The unbinding of vortex defects in the superconducting condensate with d-wave symmetry at T = 0 is shown to lead to the insulator with incommensurate spin-density-wave order .
	manualset3
168320	3	412926	7	NULL	NULL	0	NULL	 d-wave symmetry	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The unbinding of vortex defects in the superconducting condensate with d-wave symmetry at T = 0 is shown to lead to the insulator with incommensurate spin-density-wave order .
	manualset3
168321	4	412926	7	NULL	NULL	0	NULL	T = 0	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The unbinding of vortex defects in the superconducting condensate with d-wave symmetry at T = 0 is shown to lead to the insulator with incommensurate spin-density-wave order .
	manualset3
168322	5	412926	7	NULL	NULL	0	NULL	insulator	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The unbinding of vortex defects in the superconducting condensate with d-wave symmetry at T = 0 is shown to lead to the insulator with incommensurate spin-density-wave order .
	manualset3
168323	6	412926	7	NULL	NULL	0	NULL	incommensurate spin-density-wave order	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The unbinding of vortex defects in the superconducting condensate with d-wave symmetry at T = 0 is shown to lead to the insulator with incommensurate spin-density-wave order .
	manualset3
168324	1	412927	7	NULL	NULL	NULL	NULL	understanding 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The understanding of the leaching behavior of organic carbon from incinerator bottom ash is an important aspect for the control of organic carbon emissions from landfills in order to minimize their potential risk to the environment .
	manualset3
168325	2	412927	7	NULL	NULL	0	NULL	leaching behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The understanding of the leaching behavior of organic carbon from incinerator bottom ash is an important aspect for the control of organic carbon emissions from landfills in order to minimize their potential risk to the environment .
	manualset3
168326	3	412927	7	NULL	NULL	0	NULL	organic carbon	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The understanding of the leaching behavior of organic carbon from incinerator bottom ash is an important aspect for the control of organic carbon emissions from landfills in order to minimize their potential risk to the environment .
	manualset3
168327	4	412927	7	NULL	NULL	0	NULL	incinerator bottom ash	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The understanding of the leaching behavior of organic carbon from incinerator bottom ash is an important aspect for the control of organic carbon emissions from landfills in order to minimize their potential risk to the environment .
	manualset3
168328	5	412927	7	NULL	NULL	0	NULL	 control 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The understanding of the leaching behavior of organic carbon from incinerator bottom ash is an important aspect for the control of organic carbon emissions from landfills in order to minimize their potential risk to the environment .
	manualset3
168329	6	412927	7	NULL	NULL	0	NULL	organic carbon emissions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The understanding of the leaching behavior of organic carbon from incinerator bottom ash is an important aspect for the control of organic carbon emissions from landfills in order to minimize their potential risk to the environment .
	manualset3
168330	7	412927	7	NULL	NULL	0	NULL	landfills	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The understanding of the leaching behavior of organic carbon from incinerator bottom ash is an important aspect for the control of organic carbon emissions from landfills in order to minimize their potential risk to the environment .
	manualset3
168331	8	412927	7	NULL	NULL	0	NULL	potential risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The understanding of the leaching behavior of organic carbon from incinerator bottom ash is an important aspect for the control of organic carbon emissions from landfills in order to minimize their potential risk to the environment .
	manualset3
168332	9	412927	7	NULL	NULL	0	NULL	environment	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The understanding of the leaching behavior of organic carbon from incinerator bottom ash is an important aspect for the control of organic carbon emissions from landfills in order to minimize their potential risk to the environment .
	manualset3
169722	10	412927	7	NULL	NULL	0	NULL	aspect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The understanding of the leaching behavior of organic carbon from incinerator bottom ash is an important aspect for the control of organic carbon emissions from landfills in order to minimize their potential risk to the environment .
	manualset3
168333	1	412928	7	NULL	NULL	NULL	NULL	 undiscounted costs per case	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The undiscounted and discounted costs per case of diarrheal disease including sequelae were 4 , 132 and 2 , 131 , respectively .
	manualset3
168334	2	412928	7	NULL	NULL	NULL	NULL	discounted costs per case	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The undiscounted and discounted costs per case of diarrheal disease including sequelae were 4 , 132 and 2 , 131 , respectively .
	manualset3
168335	3	412928	7	NULL	NULL	0	NULL	diarrheal disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The undiscounted and discounted costs per case of diarrheal disease including sequelae were 4 , 132 and 2 , 131 , respectively .
	manualset3
168336	4	412928	7	NULL	NULL	0	NULL	 4	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The undiscounted and discounted costs per case of diarrheal disease including sequelae were 4 , 132 and 2 , 131 , respectively .
	manualset3
168337	5	412928	7	NULL	NULL	0	NULL	132	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The undiscounted and discounted costs per case of diarrheal disease including sequelae were 4 , 132 and 2 , 131 , respectively .
	manualset3
168338	6	412928	7	NULL	NULL	0	NULL	2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The undiscounted and discounted costs per case of diarrheal disease including sequelae were 4 , 132 and 2 , 131 , respectively .
	manualset3
168339	7	412928	7	NULL	NULL	0	NULL	131	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The undiscounted and discounted costs per case of diarrheal disease including sequelae were 4 , 132 and 2 , 131 , respectively .
	manualset3
169723	8	412928	7	NULL	NULL	0	NULL	sequelae	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The undiscounted and discounted costs per case of diarrheal disease including sequelae were 4 , 132 and 2 , 131 , respectively .
	manualset3
168340	1	412929	7	NULL	NULL	0	NULL	unexpected halothane concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The unexpected halothane concentration at the time of gas sampling indicated an average of 1.0 % .
	manualset3
168341	2	412929	7	NULL	NULL	0	NULL	 time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The unexpected halothane concentration at the time of gas sampling indicated an average of 1.0 % .
	manualset3
168342	3	412929	7	NULL	NULL	0	NULL	gas sampling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The unexpected halothane concentration at the time of gas sampling indicated an average of 1.0 % .
	manualset3
168343	4	412929	7	NULL	NULL	0	NULL	average	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The unexpected halothane concentration at the time of gas sampling indicated an average of 1.0 % .
	manualset3
168344	5	412929	7	NULL	NULL	0	NULL	1.0 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The unexpected halothane concentration at the time of gas sampling indicated an average of 1.0 % .
	manualset3
168345	1	412930	7	NULL	NULL	0	NULL	unfolding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The unfolding of MDH was followed using the steady-state and time resolved fluorescence methods .
	manualset3
168346	2	412930	7	NULL	NULL	0	NULL	MDH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The unfolding of MDH was followed using the steady-state and time resolved fluorescence methods .
	manualset3
168347	3	412930	7	NULL	NULL	0	NULL	steady-state and time resolved fluorescence methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The unfolding of MDH was followed using the steady-state and time resolved fluorescence methods .
	manualset3
168351	1	412931	7	NULL	NULL	0	NULL	Acta ( 1991 ) 1070 , 205-208 )	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	Acta ( 1991 ) 1070 , 205-208 ) , were used to study the effect of apo-transferrin ( apo-Tf ) in the basal chamber on 59Fe uptake from the apical surface , intracellular 59Fe distribution , and 59Fe transport into the basal chamber .
	manualset3
168352	2	412931	7	NULL	NULL	0	NULL	effect 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acta ( 1991 ) 1070 , 205-208 ) , were used to study the effect of apo-transferrin ( apo-Tf ) in the basal chamber on 59Fe uptake from the apical surface , intracellular 59Fe distribution , and 59Fe transport into the basal chamber .
	manualset3
168353	3	412931	7	NULL	NULL	0	NULL	apo-transferrin ( apo-Tf ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Acta ( 1991 ) 1070 , 205-208 ) , were used to study the effect of apo-transferrin ( apo-Tf ) in the basal chamber on 59Fe uptake from the apical surface , intracellular 59Fe distribution , and 59Fe transport into the basal chamber .
	manualset3
168354	4	412931	7	NULL	NULL	0	NULL	basal chamber	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Acta ( 1991 ) 1070 , 205-208 ) , were used to study the effect of apo-transferrin ( apo-Tf ) in the basal chamber on 59Fe uptake from the apical surface , intracellular 59Fe distribution , and 59Fe transport into the basal chamber .
	manualset3
168355	5	412931	7	NULL	NULL	0	NULL	59Fe uptake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acta ( 1991 ) 1070 , 205-208 ) , were used to study the effect of apo-transferrin ( apo-Tf ) in the basal chamber on 59Fe uptake from the apical surface , intracellular 59Fe distribution , and 59Fe transport into the basal chamber .
	manualset3
168356	6	412931	7	NULL	NULL	0	NULL	apical surface	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Acta ( 1991 ) 1070 , 205-208 ) , were used to study the effect of apo-transferrin ( apo-Tf ) in the basal chamber on 59Fe uptake from the apical surface , intracellular 59Fe distribution , and 59Fe transport into the basal chamber .
	manualset3
168357	7	412931	7	NULL	NULL	0	NULL	intracellular 59Fe distribution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acta ( 1991 ) 1070 , 205-208 ) , were used to study the effect of apo-transferrin ( apo-Tf ) in the basal chamber on 59Fe uptake from the apical surface , intracellular 59Fe distribution , and 59Fe transport into the basal chamber .
	manualset3
168358	9	412931	7	NULL	NULL	NULL	NULL	basal chamber 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Acta ( 1991 ) 1070 , 205-208 ) , were used to study the effect of apo-transferrin ( apo-Tf ) in the basal chamber on 59Fe uptake from the apical surface , intracellular 59Fe distribution , and 59Fe transport into the basal chamber .
	manualset3
168359	8	412931	7	NULL	NULL	NULL	NULL	59Fe transport	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Acta ( 1991 ) 1070 , 205-208 ) , were used to study the effect of apo-transferrin ( apo-Tf ) in the basal chamber on 59Fe uptake from the apical surface , intracellular 59Fe distribution , and 59Fe transport into the basal chamber .
	manualset3
168360	1	412932	7	NULL	NULL	0	NULL	unique problems 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The unique problems encountered in sickle patients include the need to remove peripheral vitreous if perfusing sea fans-which can bleed after vitrectomy-are present at the time of surgery .
	manualset3
168361	2	412932	7	NULL	NULL	0	NULL	sickle patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The unique problems encountered in sickle patients include the need to remove peripheral vitreous if perfusing sea fans-which can bleed after vitrectomy-are present at the time of surgery .
	manualset3
168362	3	412932	7	NULL	NULL	0	NULL	peripheral vitreous	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The unique problems encountered in sickle patients include the need to remove peripheral vitreous if perfusing sea fans-which can bleed after vitrectomy-are present at the time of surgery .
	manualset3
168363	5	412932	7	NULL	NULL	NULL	NULL	vitrectomy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The unique problems encountered in sickle patients include the need to remove peripheral vitreous if perfusing sea fans-which can bleed after vitrectomy-are present at the time of surgery .
	manualset3
168364	7	412932	7	NULL	NULL	NULL	NULL	time	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The unique problems encountered in sickle patients include the need to remove peripheral vitreous if perfusing sea fans-which can bleed after vitrectomy-are present at the time of surgery .
	manualset3
168365	8	412932	7	NULL	NULL	NULL	NULL	surgery 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The unique problems encountered in sickle patients include the need to remove peripheral vitreous if perfusing sea fans-which can bleed after vitrectomy-are present at the time of surgery .
	manualset3
168366	4	412932	7	NULL	NULL	0	NULL	perfusing sea fans	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The unique problems encountered in sickle patients include the need to remove peripheral vitreous if perfusing sea fans-which can bleed after vitrectomy-are present at the time of surgery .
	manualset3
168367	6	412932	7	NULL	NULL	NULL	NULL	present	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The unique problems encountered in sickle patients include the need to remove peripheral vitreous if perfusing sea fans-which can bleed after vitrectomy-are present at the time of surgery .
	manualset3
168368	1	412933	7	NULL	NULL	NULL	NULL	 unit cell parameters	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The unit cell parameters and corresponding changes with temperature indicate a scenario for the crystallization process .
	manualset3
168369	2	412933	7	NULL	NULL	0	NULL	changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The unit cell parameters and corresponding changes with temperature indicate a scenario for the crystallization process .
	manualset3
168370	3	412933	7	NULL	NULL	0	NULL	temperature	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The unit cell parameters and corresponding changes with temperature indicate a scenario for the crystallization process .
	manualset3
168371	4	412933	7	NULL	NULL	0	NULL	scenario 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The unit cell parameters and corresponding changes with temperature indicate a scenario for the crystallization process .
	manualset3
168372	5	412933	7	NULL	NULL	0	NULL	crystallization process 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The unit cell parameters and corresponding changes with temperature indicate a scenario for the crystallization process .
	manualset3
168373	1	412934	7	NULL	NULL	0	NULL	 universality class	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The universality class of m ( s ) = 0 is the same as that without a conserved quantity , but the universality class of nonzero m ( s ) is different .
	manualset3
168374	2	412934	7	NULL	NULL	NULL	NULL	m ( s ) = 0	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The universality class of m ( s ) = 0 is the same as that without a conserved quantity , but the universality class of nonzero m ( s ) is different .
	manualset3
168375	3	412934	7	NULL	NULL	0	NULL	conserved quantity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The universality class of m ( s ) = 0 is the same as that without a conserved quantity , but the universality class of nonzero m ( s ) is different .
	manualset3
168376	5	412934	7	NULL	NULL	NULL	NULL	nonzero m ( s )	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The universality class of m ( s ) = 0 is the same as that without a conserved quantity , but the universality class of nonzero m ( s ) is different .
	manualset3
168377	4	412934	7	NULL	NULL	0	NULL	 universality class	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The universality class of m ( s ) = 0 is the same as that without a conserved quantity , but the universality class of nonzero m ( s ) is different .
	manualset3
168378	1	412935	7	NULL	NULL	NULL	NULL	 unstable diploids	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The unstable diploids ( ery-r8 / + ) occur with a frequency equivalent to that obtained with high-efficiency ( HE ) markers , whereas the stable donor-type ( ery-r8 ) transformants occur with about five hundred times lower frequency .
	manualset3
168379	2	412935	7	NULL	NULL	NULL	NULL	 ery-r8 / +	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The unstable diploids ( ery-r8 / + ) occur with a frequency equivalent to that obtained with high-efficiency ( HE ) markers , whereas the stable donor-type ( ery-r8 ) transformants occur with about five hundred times lower frequency .
	manualset3
168380	3	412935	7	NULL	NULL	0	NULL	frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The unstable diploids ( ery-r8 / + ) occur with a frequency equivalent to that obtained with high-efficiency ( HE ) markers , whereas the stable donor-type ( ery-r8 ) transformants occur with about five hundred times lower frequency .
	manualset3
168381	4	412935	7	NULL	NULL	0	NULL	 high-efficiency ( HE ) markers	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The unstable diploids ( ery-r8 / + ) occur with a frequency equivalent to that obtained with high-efficiency ( HE ) markers , whereas the stable donor-type ( ery-r8 ) transformants occur with about five hundred times lower frequency .
	manualset3
168382	5	412935	7	NULL	NULL	0	NULL	stable donor-type ( ery-r8 ) transformants	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The unstable diploids ( ery-r8 / + ) occur with a frequency equivalent to that obtained with high-efficiency ( HE ) markers , whereas the stable donor-type ( ery-r8 ) transformants occur with about five hundred times lower frequency .
	manualset3
168383	6	412935	7	NULL	NULL	0	NULL	five hundred times	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The unstable diploids ( ery-r8 / + ) occur with a frequency equivalent to that obtained with high-efficiency ( HE ) markers , whereas the stable donor-type ( ery-r8 ) transformants occur with about five hundred times lower frequency .
	manualset3
168384	7	412935	7	NULL	NULL	0	NULL	lower frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The unstable diploids ( ery-r8 / + ) occur with a frequency equivalent to that obtained with high-efficiency ( HE ) markers , whereas the stable donor-type ( ery-r8 ) transformants occur with about five hundred times lower frequency .
	manualset3
168385	1	412936	7	NULL	NULL	0	NULL	upregulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The upregulation of interleukin 24 in dynamic 3D cultures was shown to selectively impair the viability of prostate cancer cells cultured in medium conditioned by dynamic 3D MSCs .
	manualset3
168386	2	412936	7	NULL	NULL	0	NULL	interleukin 24	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The upregulation of interleukin 24 in dynamic 3D cultures was shown to selectively impair the viability of prostate cancer cells cultured in medium conditioned by dynamic 3D MSCs .
	manualset3
168387	3	412936	7	NULL	NULL	0	NULL	dynamic 3D cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The upregulation of interleukin 24 in dynamic 3D cultures was shown to selectively impair the viability of prostate cancer cells cultured in medium conditioned by dynamic 3D MSCs .
	manualset3
168388	4	412936	7	NULL	NULL	0	NULL	viability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The upregulation of interleukin 24 in dynamic 3D cultures was shown to selectively impair the viability of prostate cancer cells cultured in medium conditioned by dynamic 3D MSCs .
	manualset3
168389	5	412936	7	NULL	NULL	0	NULL	prostate cancer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The upregulation of interleukin 24 in dynamic 3D cultures was shown to selectively impair the viability of prostate cancer cells cultured in medium conditioned by dynamic 3D MSCs .
	manualset3
168390	6	412936	7	NULL	NULL	0	NULL	medium	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The upregulation of interleukin 24 in dynamic 3D cultures was shown to selectively impair the viability of prostate cancer cells cultured in medium conditioned by dynamic 3D MSCs .
	manualset3
168391	7	412936	7	NULL	NULL	0	NULL	dynamic 3D MSCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The upregulation of interleukin 24 in dynamic 3D cultures was shown to selectively impair the viability of prostate cancer cells cultured in medium conditioned by dynamic 3D MSCs .
	manualset3
168392	1	412937	7	NULL	NULL	0	NULL	upstream mechanisms 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The upstream mechanisms of this lung injury and apoptosis have not been clearly elucidated .
	manualset3
168393	2	412937	7	NULL	NULL	0	NULL	lung injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The upstream mechanisms of this lung injury and apoptosis have not been clearly elucidated .
	manualset3
168394	3	412937	7	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The upstream mechanisms of this lung injury and apoptosis have not been clearly elucidated .
	manualset3
168395	1	412938	7	NULL	NULL	NULL	NULL	uptake	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The uptake of doxorubicin and rhodamine 123 has been quantified in LLC-PK1 and LLC-PK1 / ADR cells and compared with data obtained using other tumor cell lines commonly used as reference for studying P-gp or MRP overexpression .
	manualset3
168396	2	412938	7	NULL	NULL	0	NULL	doxorubicin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The uptake of doxorubicin and rhodamine 123 has been quantified in LLC-PK1 and LLC-PK1 / ADR cells and compared with data obtained using other tumor cell lines commonly used as reference for studying P-gp or MRP overexpression .
	manualset3
168397	3	412938	7	NULL	NULL	0	NULL	rhodamine 123	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The uptake of doxorubicin and rhodamine 123 has been quantified in LLC-PK1 and LLC-PK1 / ADR cells and compared with data obtained using other tumor cell lines commonly used as reference for studying P-gp or MRP overexpression .
	manualset3
168398	4	412938	7	NULL	NULL	0	NULL	LLC-PK1 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The uptake of doxorubicin and rhodamine 123 has been quantified in LLC-PK1 and LLC-PK1 / ADR cells and compared with data obtained using other tumor cell lines commonly used as reference for studying P-gp or MRP overexpression .
	manualset3
168399	5	412938	7	NULL	NULL	0	NULL	LLC-PK1 / ADR cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The uptake of doxorubicin and rhodamine 123 has been quantified in LLC-PK1 and LLC-PK1 / ADR cells and compared with data obtained using other tumor cell lines commonly used as reference for studying P-gp or MRP overexpression .
	manualset3
168400	6	412938	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The uptake of doxorubicin and rhodamine 123 has been quantified in LLC-PK1 and LLC-PK1 / ADR cells and compared with data obtained using other tumor cell lines commonly used as reference for studying P-gp or MRP overexpression .
	manualset3
168401	7	412938	7	NULL	NULL	0	NULL	tumor cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The uptake of doxorubicin and rhodamine 123 has been quantified in LLC-PK1 and LLC-PK1 / ADR cells and compared with data obtained using other tumor cell lines commonly used as reference for studying P-gp or MRP overexpression .
	manualset3
168402	8	412938	7	NULL	NULL	0	NULL	reference	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The uptake of doxorubicin and rhodamine 123 has been quantified in LLC-PK1 and LLC-PK1 / ADR cells and compared with data obtained using other tumor cell lines commonly used as reference for studying P-gp or MRP overexpression .
	manualset3
168403	9	412938	7	NULL	NULL	0	NULL	P-gp overexpression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The uptake of doxorubicin and rhodamine 123 has been quantified in LLC-PK1 and LLC-PK1 / ADR cells and compared with data obtained using other tumor cell lines commonly used as reference for studying P-gp or MRP overexpression .
	manualset3
168404	10	412938	7	NULL	NULL	0	NULL	MRP overexpression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The uptake of doxorubicin and rhodamine 123 has been quantified in LLC-PK1 and LLC-PK1 / ADR cells and compared with data obtained using other tumor cell lines commonly used as reference for studying P-gp or MRP overexpression .
	manualset3
171364	11	412938	7	NULL	NULL	0	NULL	studying	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The uptake of doxorubicin and rhodamine 123 has been quantified in LLC-PK1 and LLC-PK1 / ADR cells and compared with data obtained using other tumor cell lines commonly used as reference for studying P-gp or MRP overexpression .
	manualset3
168405	1	412939	7	NULL	NULL	0	NULL	uraA locus 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The uraA locus and homologous recombination in Mycobacterium bovis BCG .
	manualset3
168406	2	412939	7	NULL	NULL	0	NULL	homologous recombination	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The uraA locus and homologous recombination in Mycobacterium bovis BCG .
	manualset3
168407	3	412939	7	NULL	NULL	0	NULL	Mycobacterium bovis BCG	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The uraA locus and homologous recombination in Mycobacterium bovis BCG .
	manualset3
168408	1	412940	7	NULL	NULL	0	NULL	urethral syndrome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The urethral syndrome , the author concludes , is therefore based on recognized anatomical factors .
	manualset3
168409	2	412940	7	NULL	NULL	0	NULL	 author	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The urethral syndrome , the author concludes , is therefore based on recognized anatomical factors .
	manualset3
168410	3	412940	7	NULL	NULL	0	NULL	recognized anatomical factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The urethral syndrome , the author concludes , is therefore based on recognized anatomical factors .
	manualset3
168411	1	412941	7	NULL	NULL	0	NULL	Actin-binding proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Actin-binding proteins required for reliable chromosome segregation in mitosis .
	manualset3
168412	2	412941	7	NULL	NULL	0	NULL	chromosome segregation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Actin-binding proteins required for reliable chromosome segregation in mitosis .
	manualset3
168413	3	412941	7	NULL	NULL	0	NULL	mitosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Actin-binding proteins required for reliable chromosome segregation in mitosis .
	manualset3
168414	1	412942	7	NULL	NULL	0	NULL	urinary excretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of 6-keto-PGF1a was similar in both groups ( 249.8 + / - 18.5 , mean + / - SEM , and 262.7 + / - 35.0 pg 6-keto-PGF1a / mmol of creatinine for BSM and BNSM , respectively , on the first day of life ; 109.4 + / - 18.6 and 133.3 + / - 18.5 pg/mmol for BSM and BNSM , respectively , on the third or fourth day of life ) .
	manualset3
168415	2	412942	7	NULL	NULL	0	NULL	6-keto-PGF1a	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of 6-keto-PGF1a was similar in both groups ( 249.8 + / - 18.5 , mean + / - SEM , and 262.7 + / - 35.0 pg 6-keto-PGF1a / mmol of creatinine for BSM and BNSM , respectively , on the first day of life ; 109.4 + / - 18.6 and 133.3 + / - 18.5 pg/mmol for BSM and BNSM , respectively , on the third or fourth day of life ) .
	manualset3
168416	3	412942	7	NULL	NULL	0	NULL	groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of 6-keto-PGF1a was similar in both groups ( 249.8 + / - 18.5 , mean + / - SEM , and 262.7 + / - 35.0 pg 6-keto-PGF1a / mmol of creatinine for BSM and BNSM , respectively , on the first day of life ; 109.4 + / - 18.6 and 133.3 + / - 18.5 pg/mmol for BSM and BNSM , respectively , on the third or fourth day of life ) .
	manualset3
168417	4	412942	7	NULL	NULL	0	NULL	249.8 + / - 18.5 , mean + / - SEM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of 6-keto-PGF1a was similar in both groups ( 249.8 + / - 18.5 , mean + / - SEM , and 262.7 + / - 35.0 pg 6-keto-PGF1a / mmol of creatinine for BSM and BNSM , respectively , on the first day of life ; 109.4 + / - 18.6 and 133.3 + / - 18.5 pg/mmol for BSM and BNSM , respectively , on the third or fourth day of life ) .
	manualset3
168418	5	412942	7	NULL	NULL	0	NULL	262.7 + / - 35.0 pg 6-keto-PGF1a / mmol	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of 6-keto-PGF1a was similar in both groups ( 249.8 + / - 18.5 , mean + / - SEM , and 262.7 + / - 35.0 pg 6-keto-PGF1a / mmol of creatinine for BSM and BNSM , respectively , on the first day of life ; 109.4 + / - 18.6 and 133.3 + / - 18.5 pg/mmol for BSM and BNSM , respectively , on the third or fourth day of life ) .
	manualset3
168419	6	412942	7	NULL	NULL	0	NULL	creatinine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of 6-keto-PGF1a was similar in both groups ( 249.8 + / - 18.5 , mean + / - SEM , and 262.7 + / - 35.0 pg 6-keto-PGF1a / mmol of creatinine for BSM and BNSM , respectively , on the first day of life ; 109.4 + / - 18.6 and 133.3 + / - 18.5 pg/mmol for BSM and BNSM , respectively , on the third or fourth day of life ) .
	manualset3
168420	7	412942	7	NULL	NULL	0	NULL	 BSM	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of 6-keto-PGF1a was similar in both groups ( 249.8 + / - 18.5 , mean + / - SEM , and 262.7 + / - 35.0 pg 6-keto-PGF1a / mmol of creatinine for BSM and BNSM , respectively , on the first day of life ; 109.4 + / - 18.6 and 133.3 + / - 18.5 pg/mmol for BSM and BNSM , respectively , on the third or fourth day of life ) .
	manualset3
168421	8	412942	7	NULL	NULL	0	NULL	BNSM	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of 6-keto-PGF1a was similar in both groups ( 249.8 + / - 18.5 , mean + / - SEM , and 262.7 + / - 35.0 pg 6-keto-PGF1a / mmol of creatinine for BSM and BNSM , respectively , on the first day of life ; 109.4 + / - 18.6 and 133.3 + / - 18.5 pg/mmol for BSM and BNSM , respectively , on the third or fourth day of life ) .
	manualset3
168422	9	412942	7	NULL	NULL	0	NULL	first day	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of 6-keto-PGF1a was similar in both groups ( 249.8 + / - 18.5 , mean + / - SEM , and 262.7 + / - 35.0 pg 6-keto-PGF1a / mmol of creatinine for BSM and BNSM , respectively , on the first day of life ; 109.4 + / - 18.6 and 133.3 + / - 18.5 pg/mmol for BSM and BNSM , respectively , on the third or fourth day of life ) .
	manualset3
168423	10	412942	7	NULL	NULL	0	NULL	life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of 6-keto-PGF1a was similar in both groups ( 249.8 + / - 18.5 , mean + / - SEM , and 262.7 + / - 35.0 pg 6-keto-PGF1a / mmol of creatinine for BSM and BNSM , respectively , on the first day of life ; 109.4 + / - 18.6 and 133.3 + / - 18.5 pg/mmol for BSM and BNSM , respectively , on the third or fourth day of life ) .
	manualset3
168424	11	412942	7	NULL	NULL	0	NULL	109.4 + / - 18.6	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of 6-keto-PGF1a was similar in both groups ( 249.8 + / - 18.5 , mean + / - SEM , and 262.7 + / - 35.0 pg 6-keto-PGF1a / mmol of creatinine for BSM and BNSM , respectively , on the first day of life ; 109.4 + / - 18.6 and 133.3 + / - 18.5 pg/mmol for BSM and BNSM , respectively , on the third or fourth day of life ) .
	manualset3
168425	12	412942	7	NULL	NULL	0	NULL	133.3 + / - 18.5 pg/mmol	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of 6-keto-PGF1a was similar in both groups ( 249.8 + / - 18.5 , mean + / - SEM , and 262.7 + / - 35.0 pg 6-keto-PGF1a / mmol of creatinine for BSM and BNSM , respectively , on the first day of life ; 109.4 + / - 18.6 and 133.3 + / - 18.5 pg/mmol for BSM and BNSM , respectively , on the third or fourth day of life ) .
	manualset3
168426	13	412942	7	NULL	NULL	0	NULL	BSM	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of 6-keto-PGF1a was similar in both groups ( 249.8 + / - 18.5 , mean + / - SEM , and 262.7 + / - 35.0 pg 6-keto-PGF1a / mmol of creatinine for BSM and BNSM , respectively , on the first day of life ; 109.4 + / - 18.6 and 133.3 + / - 18.5 pg/mmol for BSM and BNSM , respectively , on the third or fourth day of life ) .
	manualset3
168427	14	412942	7	NULL	NULL	0	NULL	BNSM	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of 6-keto-PGF1a was similar in both groups ( 249.8 + / - 18.5 , mean + / - SEM , and 262.7 + / - 35.0 pg 6-keto-PGF1a / mmol of creatinine for BSM and BNSM , respectively , on the first day of life ; 109.4 + / - 18.6 and 133.3 + / - 18.5 pg/mmol for BSM and BNSM , respectively , on the third or fourth day of life ) .
	manualset3
168428	15	412942	7	NULL	NULL	0	NULL	 third day	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of 6-keto-PGF1a was similar in both groups ( 249.8 + / - 18.5 , mean + / - SEM , and 262.7 + / - 35.0 pg 6-keto-PGF1a / mmol of creatinine for BSM and BNSM , respectively , on the first day of life ; 109.4 + / - 18.6 and 133.3 + / - 18.5 pg/mmol for BSM and BNSM , respectively , on the third or fourth day of life ) .
	manualset3
168429	16	412942	7	NULL	NULL	0	NULL	fourth day 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of 6-keto-PGF1a was similar in both groups ( 249.8 + / - 18.5 , mean + / - SEM , and 262.7 + / - 35.0 pg 6-keto-PGF1a / mmol of creatinine for BSM and BNSM , respectively , on the first day of life ; 109.4 + / - 18.6 and 133.3 + / - 18.5 pg/mmol for BSM and BNSM , respectively , on the third or fourth day of life ) .
	manualset3
168430	17	412942	7	NULL	NULL	0	NULL	life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of 6-keto-PGF1a was similar in both groups ( 249.8 + / - 18.5 , mean + / - SEM , and 262.7 + / - 35.0 pg 6-keto-PGF1a / mmol of creatinine for BSM and BNSM , respectively , on the first day of life ; 109.4 + / - 18.6 and 133.3 + / - 18.5 pg/mmol for BSM and BNSM , respectively , on the third or fourth day of life ) .
	manualset3
168431	1	412943	7	NULL	NULL	0	NULL	urinary excretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of hyaluronic acid ( HA ) ( mg/day ) was significantly increased ( P & lt ; 0.01 ) in ALS patients compared with that of control subjects , and there was a significant positive correlation between the excreted amount of HA and the duration of illness in advanced ALS patients with a duration of more than 2 years from clinical onset ( r = 0.72 , P & lt ; 0.02 ) .
	manualset3
168432	2	412943	7	NULL	NULL	0	NULL	hyaluronic acid ( HA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of hyaluronic acid ( HA ) ( mg/day ) was significantly increased ( P & lt ; 0.01 ) in ALS patients compared with that of control subjects , and there was a significant positive correlation between the excreted amount of HA and the duration of illness in advanced ALS patients with a duration of more than 2 years from clinical onset ( r = 0.72 , P & lt ; 0.02 ) .
	manualset3
168433	3	412943	7	NULL	NULL	0	NULL	mg/day	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of hyaluronic acid ( HA ) ( mg/day ) was significantly increased ( P & lt ; 0.01 ) in ALS patients compared with that of control subjects , and there was a significant positive correlation between the excreted amount of HA and the duration of illness in advanced ALS patients with a duration of more than 2 years from clinical onset ( r = 0.72 , P & lt ; 0.02 ) .
	manualset3
168434	4	412943	7	NULL	NULL	0	NULL	P & lt ; 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of hyaluronic acid ( HA ) ( mg/day ) was significantly increased ( P & lt ; 0.01 ) in ALS patients compared with that of control subjects , and there was a significant positive correlation between the excreted amount of HA and the duration of illness in advanced ALS patients with a duration of more than 2 years from clinical onset ( r = 0.72 , P & lt ; 0.02 ) .
	manualset3
168435	5	412943	7	NULL	NULL	0	NULL	ALS patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of hyaluronic acid ( HA ) ( mg/day ) was significantly increased ( P & lt ; 0.01 ) in ALS patients compared with that of control subjects , and there was a significant positive correlation between the excreted amount of HA and the duration of illness in advanced ALS patients with a duration of more than 2 years from clinical onset ( r = 0.72 , P & lt ; 0.02 ) .
	manualset3
168436	6	412943	7	NULL	NULL	0	NULL	control subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of hyaluronic acid ( HA ) ( mg/day ) was significantly increased ( P & lt ; 0.01 ) in ALS patients compared with that of control subjects , and there was a significant positive correlation between the excreted amount of HA and the duration of illness in advanced ALS patients with a duration of more than 2 years from clinical onset ( r = 0.72 , P & lt ; 0.02 ) .
	manualset3
168437	7	412943	7	NULL	NULL	0	NULL	positive correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of hyaluronic acid ( HA ) ( mg/day ) was significantly increased ( P & lt ; 0.01 ) in ALS patients compared with that of control subjects , and there was a significant positive correlation between the excreted amount of HA and the duration of illness in advanced ALS patients with a duration of more than 2 years from clinical onset ( r = 0.72 , P & lt ; 0.02 ) .
	manualset3
168439	8	412943	7	NULL	NULL	0	NULL	excreted amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of hyaluronic acid ( HA ) ( mg/day ) was significantly increased ( P & lt ; 0.01 ) in ALS patients compared with that of control subjects , and there was a significant positive correlation between the excreted amount of HA and the duration of illness in advanced ALS patients with a duration of more than 2 years from clinical onset ( r = 0.72 , P & lt ; 0.02 ) .
	manualset3
168440	9	412943	7	NULL	NULL	0	NULL	HA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of hyaluronic acid ( HA ) ( mg/day ) was significantly increased ( P & lt ; 0.01 ) in ALS patients compared with that of control subjects , and there was a significant positive correlation between the excreted amount of HA and the duration of illness in advanced ALS patients with a duration of more than 2 years from clinical onset ( r = 0.72 , P & lt ; 0.02 ) .
	manualset3
168441	10	412943	7	NULL	NULL	0	NULL	duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of hyaluronic acid ( HA ) ( mg/day ) was significantly increased ( P & lt ; 0.01 ) in ALS patients compared with that of control subjects , and there was a significant positive correlation between the excreted amount of HA and the duration of illness in advanced ALS patients with a duration of more than 2 years from clinical onset ( r = 0.72 , P & lt ; 0.02 ) .
	manualset3
168442	11	412943	7	NULL	NULL	0	NULL	illness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of hyaluronic acid ( HA ) ( mg/day ) was significantly increased ( P & lt ; 0.01 ) in ALS patients compared with that of control subjects , and there was a significant positive correlation between the excreted amount of HA and the duration of illness in advanced ALS patients with a duration of more than 2 years from clinical onset ( r = 0.72 , P & lt ; 0.02 ) .
	manualset3
168443	12	412943	7	NULL	NULL	0	NULL	advanced ALS patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of hyaluronic acid ( HA ) ( mg/day ) was significantly increased ( P & lt ; 0.01 ) in ALS patients compared with that of control subjects , and there was a significant positive correlation between the excreted amount of HA and the duration of illness in advanced ALS patients with a duration of more than 2 years from clinical onset ( r = 0.72 , P & lt ; 0.02 ) .
	manualset3
168444	13	412943	7	NULL	NULL	0	NULL	duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of hyaluronic acid ( HA ) ( mg/day ) was significantly increased ( P & lt ; 0.01 ) in ALS patients compared with that of control subjects , and there was a significant positive correlation between the excreted amount of HA and the duration of illness in advanced ALS patients with a duration of more than 2 years from clinical onset ( r = 0.72 , P & lt ; 0.02 ) .
	manualset3
168445	14	412943	7	NULL	NULL	0	NULL	2 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of hyaluronic acid ( HA ) ( mg/day ) was significantly increased ( P & lt ; 0.01 ) in ALS patients compared with that of control subjects , and there was a significant positive correlation between the excreted amount of HA and the duration of illness in advanced ALS patients with a duration of more than 2 years from clinical onset ( r = 0.72 , P & lt ; 0.02 ) .
	manualset3
168446	15	412943	7	NULL	NULL	0	NULL	clinical onset	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of hyaluronic acid ( HA ) ( mg/day ) was significantly increased ( P & lt ; 0.01 ) in ALS patients compared with that of control subjects , and there was a significant positive correlation between the excreted amount of HA and the duration of illness in advanced ALS patients with a duration of more than 2 years from clinical onset ( r = 0.72 , P & lt ; 0.02 ) .
	manualset3
168447	16	412943	7	NULL	NULL	0	NULL	r = 0.72 , P & lt ; 0.02 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The urinary excretion of hyaluronic acid ( HA ) ( mg/day ) was significantly increased ( P & lt ; 0.01 ) in ALS patients compared with that of control subjects , and there was a significant positive correlation between the excreted amount of HA and the duration of illness in advanced ALS patients with a duration of more than 2 years from clinical onset ( r = 0.72 , P & lt ; 0.02 ) .
	manualset3
168448	1	412944	7	NULL	NULL	NULL	NULL	 use of I-SCD	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of I-SCD in oligospermia and OTA Syndrome is therefore indicated , both diagnostically and therapeutically .
	manualset3
168449	2	412944	7	NULL	NULL	0	NULL	oligospermia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of I-SCD in oligospermia and OTA Syndrome is therefore indicated , both diagnostically and therapeutically .
	manualset3
168450	3	412944	7	NULL	NULL	0	NULL	OTA Syndrome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of I-SCD in oligospermia and OTA Syndrome is therefore indicated , both diagnostically and therapeutically .
	manualset3
168451	1	412945	7	NULL	NULL	NULL	NULL	use of N-alkoxycarbonyl derivatives	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of N-alkoxycarbonyl derivatives of 2-amino-2-deoxy-D-glucose as donors in glycosylation reactions .
	manualset3
168452	2	412945	7	NULL	NULL	0	NULL	2-amino-2-deoxy-D-glucose	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of N-alkoxycarbonyl derivatives of 2-amino-2-deoxy-D-glucose as donors in glycosylation reactions .
	manualset3
168453	3	412945	7	NULL	NULL	0	NULL	donors	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of N-alkoxycarbonyl derivatives of 2-amino-2-deoxy-D-glucose as donors in glycosylation reactions .
	manualset3
168454	4	412945	7	NULL	NULL	0	NULL	glycosylation reactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of N-alkoxycarbonyl derivatives of 2-amino-2-deoxy-D-glucose as donors in glycosylation reactions .
	manualset3
168455	1	412946	7	NULL	NULL	NULL	NULL	use of NaOCl	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of NaOCl as an endodontic irrigant lowers the bond strength of resin cements but this can be reversed by the use of 10 % sodium ascorbate for 10 min .
	manualset3
168456	2	412946	7	NULL	NULL	0	NULL	endodontic irrigant 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of NaOCl as an endodontic irrigant lowers the bond strength of resin cements but this can be reversed by the use of 10 % sodium ascorbate for 10 min .
	manualset3
168457	3	412946	7	NULL	NULL	0	NULL	bond strength 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of NaOCl as an endodontic irrigant lowers the bond strength of resin cements but this can be reversed by the use of 10 % sodium ascorbate for 10 min .
	manualset3
168458	4	412946	7	NULL	NULL	0	NULL	resin cements	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of NaOCl as an endodontic irrigant lowers the bond strength of resin cements but this can be reversed by the use of 10 % sodium ascorbate for 10 min .
	manualset3
168459	5	412946	7	NULL	NULL	0	NULL	10 % sodium ascorbate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of NaOCl as an endodontic irrigant lowers the bond strength of resin cements but this can be reversed by the use of 10 % sodium ascorbate for 10 min .
	manualset3
168460	6	412946	7	NULL	NULL	0	NULL	10 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of NaOCl as an endodontic irrigant lowers the bond strength of resin cements but this can be reversed by the use of 10 % sodium ascorbate for 10 min .
	manualset3
168461	1	412947	7	NULL	NULL	NULL	NULL	use of YAG-tipped contact laser	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of YAG-tipped contact laser in removing orbital lymphangiomas .
	manualset3
168462	2	412947	7	NULL	NULL	0	NULL	orbital lymphangiomas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of YAG-tipped contact laser in removing orbital lymphangiomas .
	manualset3
168463	1	412948	7	NULL	NULL	NULL	NULL	 use of behavior scale	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of a behavior scale permitted to conclude that pimozide improves social integration in the Socio-familial milieu .
	manualset3
168464	2	412948	7	NULL	NULL	0	NULL	pimozide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of a behavior scale permitted to conclude that pimozide improves social integration in the Socio-familial milieu .
	manualset3
168465	3	412948	7	NULL	NULL	0	NULL	social integration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of a behavior scale permitted to conclude that pimozide improves social integration in the Socio-familial milieu .
	manualset3
168466	4	412948	7	NULL	NULL	0	NULL	Socio-familial milieu	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of a behavior scale permitted to conclude that pimozide improves social integration in the Socio-familial milieu .
	manualset3
168467	1	412949	7	NULL	NULL	NULL	NULL	use of third extrastimulus	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of a third extrastimulus increased the yield of inducible ventricular tachycardia by 37 % in patients with a history of sustained ventricular tachycardia and by 25 % in patients with a history of sudden cardiac death .
	manualset3
168468	2	412949	7	NULL	NULL	0	NULL	yield 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of a third extrastimulus increased the yield of inducible ventricular tachycardia by 37 % in patients with a history of sustained ventricular tachycardia and by 25 % in patients with a history of sudden cardiac death .
	manualset3
168469	3	412949	7	NULL	NULL	0	NULL	inducible ventricular tachycardia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of a third extrastimulus increased the yield of inducible ventricular tachycardia by 37 % in patients with a history of sustained ventricular tachycardia and by 25 % in patients with a history of sudden cardiac death .
	manualset3
168470	4	412949	7	NULL	NULL	0	NULL	37 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of a third extrastimulus increased the yield of inducible ventricular tachycardia by 37 % in patients with a history of sustained ventricular tachycardia and by 25 % in patients with a history of sudden cardiac death .
	manualset3
168471	5	412949	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of a third extrastimulus increased the yield of inducible ventricular tachycardia by 37 % in patients with a history of sustained ventricular tachycardia and by 25 % in patients with a history of sudden cardiac death .
	manualset3
168472	6	412949	7	NULL	NULL	0	NULL	history 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of a third extrastimulus increased the yield of inducible ventricular tachycardia by 37 % in patients with a history of sustained ventricular tachycardia and by 25 % in patients with a history of sudden cardiac death .
	manualset3
168473	7	412949	7	NULL	NULL	0	NULL	sustained ventricular tachycardia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of a third extrastimulus increased the yield of inducible ventricular tachycardia by 37 % in patients with a history of sustained ventricular tachycardia and by 25 % in patients with a history of sudden cardiac death .
	manualset3
168474	8	412949	7	NULL	NULL	0	NULL	25 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of a third extrastimulus increased the yield of inducible ventricular tachycardia by 37 % in patients with a history of sustained ventricular tachycardia and by 25 % in patients with a history of sudden cardiac death .
	manualset3
168475	9	412949	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of a third extrastimulus increased the yield of inducible ventricular tachycardia by 37 % in patients with a history of sustained ventricular tachycardia and by 25 % in patients with a history of sudden cardiac death .
	manualset3
168476	10	412949	7	NULL	NULL	0	NULL	history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of a third extrastimulus increased the yield of inducible ventricular tachycardia by 37 % in patients with a history of sustained ventricular tachycardia and by 25 % in patients with a history of sudden cardiac death .
	manualset3
168477	11	412949	7	NULL	NULL	0	NULL	sudden cardiac death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of a third extrastimulus increased the yield of inducible ventricular tachycardia by 37 % in patients with a history of sustained ventricular tachycardia and by 25 % in patients with a history of sudden cardiac death .
	manualset3
168478	1	412950	7	NULL	NULL	0	NULL	Actin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Actin works in concert with myosin I to regulate the transcription of ribosomal genes in the nucleolus .
	manualset3
168479	2	412950	7	NULL	NULL	0	NULL	myosin I 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Actin works in concert with myosin I to regulate the transcription of ribosomal genes in the nucleolus .
	manualset3
168480	3	412950	7	NULL	NULL	0	NULL	transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Actin works in concert with myosin I to regulate the transcription of ribosomal genes in the nucleolus .
	manualset3
168481	4	412950	7	NULL	NULL	0	NULL	ribosomal genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Actin works in concert with myosin I to regulate the transcription of ribosomal genes in the nucleolus .
	manualset3
168482	5	412950	7	NULL	NULL	0	NULL	nucleolus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Actin works in concert with myosin I to regulate the transcription of ribosomal genes in the nucleolus .
	manualset3
168483	1	412951	7	NULL	NULL	NULL	NULL	use of automated solid-phase extraction	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of automated solid-phase extraction and stable labeled internal standards permitted the robust determination of ethenodeoxyadenosine contained in crude DNA hydrolysates from untreated rodent and human tissues at levels on the order of one adduct in 10 ( 8 ) normal nucleotides from 100 microg of DNA .
	manualset3
168484	2	412951	7	NULL	NULL	0	NULL	stable labeled internal standards	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of automated solid-phase extraction and stable labeled internal standards permitted the robust determination of ethenodeoxyadenosine contained in crude DNA hydrolysates from untreated rodent and human tissues at levels on the order of one adduct in 10 ( 8 ) normal nucleotides from 100 microg of DNA .
	manualset3
168485	3	412951	7	NULL	NULL	0	NULL	determination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of automated solid-phase extraction and stable labeled internal standards permitted the robust determination of ethenodeoxyadenosine contained in crude DNA hydrolysates from untreated rodent and human tissues at levels on the order of one adduct in 10 ( 8 ) normal nucleotides from 100 microg of DNA .
	manualset3
168486	4	412951	7	NULL	NULL	0	NULL	ethenodeoxyadenosine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of automated solid-phase extraction and stable labeled internal standards permitted the robust determination of ethenodeoxyadenosine contained in crude DNA hydrolysates from untreated rodent and human tissues at levels on the order of one adduct in 10 ( 8 ) normal nucleotides from 100 microg of DNA .
	manualset3
168487	5	412951	7	NULL	NULL	0	NULL	crude DNA hydrolysates	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of automated solid-phase extraction and stable labeled internal standards permitted the robust determination of ethenodeoxyadenosine contained in crude DNA hydrolysates from untreated rodent and human tissues at levels on the order of one adduct in 10 ( 8 ) normal nucleotides from 100 microg of DNA .
	manualset3
168488	6	412951	7	NULL	NULL	0	NULL	untreated rodent tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of automated solid-phase extraction and stable labeled internal standards permitted the robust determination of ethenodeoxyadenosine contained in crude DNA hydrolysates from untreated rodent and human tissues at levels on the order of one adduct in 10 ( 8 ) normal nucleotides from 100 microg of DNA .
	manualset3
168489	7	412951	7	NULL	NULL	0	NULL	human tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of automated solid-phase extraction and stable labeled internal standards permitted the robust determination of ethenodeoxyadenosine contained in crude DNA hydrolysates from untreated rodent and human tissues at levels on the order of one adduct in 10 ( 8 ) normal nucleotides from 100 microg of DNA .
	manualset3
168490	8	412951	7	NULL	NULL	0	NULL	levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of automated solid-phase extraction and stable labeled internal standards permitted the robust determination of ethenodeoxyadenosine contained in crude DNA hydrolysates from untreated rodent and human tissues at levels on the order of one adduct in 10 ( 8 ) normal nucleotides from 100 microg of DNA .
	manualset3
168491	9	412951	7	NULL	NULL	0	NULL	order	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of automated solid-phase extraction and stable labeled internal standards permitted the robust determination of ethenodeoxyadenosine contained in crude DNA hydrolysates from untreated rodent and human tissues at levels on the order of one adduct in 10 ( 8 ) normal nucleotides from 100 microg of DNA .
	manualset3
168492	10	412951	7	NULL	NULL	0	NULL	one adduct	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of automated solid-phase extraction and stable labeled internal standards permitted the robust determination of ethenodeoxyadenosine contained in crude DNA hydrolysates from untreated rodent and human tissues at levels on the order of one adduct in 10 ( 8 ) normal nucleotides from 100 microg of DNA .
	manualset3
168493	11	412951	7	NULL	NULL	0	NULL	10 ( 8 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of automated solid-phase extraction and stable labeled internal standards permitted the robust determination of ethenodeoxyadenosine contained in crude DNA hydrolysates from untreated rodent and human tissues at levels on the order of one adduct in 10 ( 8 ) normal nucleotides from 100 microg of DNA .
	manualset3
168494	12	412951	7	NULL	NULL	0	NULL	nucleotides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of automated solid-phase extraction and stable labeled internal standards permitted the robust determination of ethenodeoxyadenosine contained in crude DNA hydrolysates from untreated rodent and human tissues at levels on the order of one adduct in 10 ( 8 ) normal nucleotides from 100 microg of DNA .
	manualset3
168495	13	412951	7	NULL	NULL	0	NULL	100 microg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of automated solid-phase extraction and stable labeled internal standards permitted the robust determination of ethenodeoxyadenosine contained in crude DNA hydrolysates from untreated rodent and human tissues at levels on the order of one adduct in 10 ( 8 ) normal nucleotides from 100 microg of DNA .
	manualset3
168496	14	412951	7	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of automated solid-phase extraction and stable labeled internal standards permitted the robust determination of ethenodeoxyadenosine contained in crude DNA hydrolysates from untreated rodent and human tissues at levels on the order of one adduct in 10 ( 8 ) normal nucleotides from 100 microg of DNA .
	manualset3
168497	1	412952	7	NULL	NULL	NULL	NULL	use of bromocriptine	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of bromocriptine in parkinsonism after carbon monoxide poisoning .
	manualset3
168498	2	412952	7	NULL	NULL	0	NULL	parkinsonism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of bromocriptine in parkinsonism after carbon monoxide poisoning .
	manualset3
168499	3	412952	7	NULL	NULL	0	NULL	carbon monoxide poisoning	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of bromocriptine in parkinsonism after carbon monoxide poisoning .
	manualset3
168500	1	412953	7	NULL	NULL	NULL	NULL	use of chemotherapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of chemotherapy , hormonal therapy , and immunotherapy changed little .
	manualset3
168501	2	412953	7	NULL	NULL	0	NULL	hormonal therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of chemotherapy , hormonal therapy , and immunotherapy changed little .
	manualset3
168502	3	412953	7	NULL	NULL	0	NULL	immunotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of chemotherapy , hormonal therapy , and immunotherapy changed little .
	manualset3
168503	1	412954	7	NULL	NULL	NULL	NULL	use of color sorting	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of color sorting after kilning showed higher concentrations of each mycotoxin in the discolored groats .
	manualset3
168504	2	412954	7	NULL	NULL	0	NULL	kilning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of color sorting after kilning showed higher concentrations of each mycotoxin in the discolored groats .
	manualset3
168505	3	412954	7	NULL	NULL	NULL	NULL	higher concentrations	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of color sorting after kilning showed higher concentrations of each mycotoxin in the discolored groats .
	manualset3
168506	4	412954	7	NULL	NULL	0	NULL	mycotoxin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of color sorting after kilning showed higher concentrations of each mycotoxin in the discolored groats .
	manualset3
168507	5	412954	7	NULL	NULL	0	NULL	discolored groats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of color sorting after kilning showed higher concentrations of each mycotoxin in the discolored groats .
	manualset3
168508	1	412955	7	NULL	NULL	NULL	NULL	use of diagnostic laparoscopy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of diagnostic laparoscopy supported by laparoscopic ultrasonography in the assessment of pancreatic cancer .
	manualset3
168509	2	412955	7	NULL	NULL	NULL	NULL	laparoscopic ultrasonography	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of diagnostic laparoscopy supported by laparoscopic ultrasonography in the assessment of pancreatic cancer .
	manualset3
168510	3	412955	7	NULL	NULL	0	NULL	assessment 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of diagnostic laparoscopy supported by laparoscopic ultrasonography in the assessment of pancreatic cancer .
	manualset3
168511	4	412955	7	NULL	NULL	0	NULL	pancreatic cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of diagnostic laparoscopy supported by laparoscopic ultrasonography in the assessment of pancreatic cancer .
	manualset3
168512	1	412956	7	NULL	NULL	NULL	NULL	use of ethnography	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of ethnography and narrative interviews in a study of ` cultures of dance ' .
	manualset3
168513	2	412956	7	NULL	NULL	NULL	NULL	 narrative interviews	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of ethnography and narrative interviews in a study of ` cultures of dance ' .
	manualset3
168514	3	412956	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of ethnography and narrative interviews in a study of ` cultures of dance ' .
	manualset3
168515	4	412956	7	NULL	NULL	0	NULL	cultures of dance	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of ethnography and narrative interviews in a study of ` cultures of dance ' .
	manualset3
168516	1	412957	7	NULL	NULL	NULL	NULL	use of exogenous growth factors	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of exogenous growth factors on diabetic wounds has been found to stimulate fibroblast proliferation and facilitate wound healing .
	manualset3
168517	2	412957	7	NULL	NULL	0	NULL	diabetic wounds	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of exogenous growth factors on diabetic wounds has been found to stimulate fibroblast proliferation and facilitate wound healing .
	manualset3
168518	3	412957	7	NULL	NULL	0	NULL	fibroblast proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of exogenous growth factors on diabetic wounds has been found to stimulate fibroblast proliferation and facilitate wound healing .
	manualset3
168519	4	412957	7	NULL	NULL	0	NULL	wound healing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of exogenous growth factors on diabetic wounds has been found to stimulate fibroblast proliferation and facilitate wound healing .
	manualset3
168520	1	412958	7	NULL	NULL	NULL	NULL	use of extracts 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of extracts in the skin test and the additional use of IgE testing still represent the current basis for the diagnostic work-up .
	manualset3
168521	2	412958	7	NULL	NULL	0	NULL	skin test	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of extracts in the skin test and the additional use of IgE testing still represent the current basis for the diagnostic work-up .
	manualset3
168522	3	412958	7	NULL	NULL	0	NULL	IgE testing 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of extracts in the skin test and the additional use of IgE testing still represent the current basis for the diagnostic work-up .
	manualset3
168523	4	412958	7	NULL	NULL	0	NULL	basis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of extracts in the skin test and the additional use of IgE testing still represent the current basis for the diagnostic work-up .
	manualset3
168524	5	412958	7	NULL	NULL	0	NULL	diagnostic work-up	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of extracts in the skin test and the additional use of IgE testing still represent the current basis for the diagnostic work-up .
	manualset3
168525	1	412959	7	NULL	NULL	NULL	NULL	use of ganciclovir	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of ganciclovir in the treatment of cytomegalovirus ( CMV ) retinitis in patients with acquired immunodeficiency syndrome ( AIDS ) is limited by marrow toxicity and by the development of resistance to this agent in CMV strains capable of causing progressive disease .
	manualset3
168526	2	412959	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of ganciclovir in the treatment of cytomegalovirus ( CMV ) retinitis in patients with acquired immunodeficiency syndrome ( AIDS ) is limited by marrow toxicity and by the development of resistance to this agent in CMV strains capable of causing progressive disease .
	manualset3
168527	3	412959	7	NULL	NULL	0	NULL	cytomegalovirus ( CMV ) retinitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of ganciclovir in the treatment of cytomegalovirus ( CMV ) retinitis in patients with acquired immunodeficiency syndrome ( AIDS ) is limited by marrow toxicity and by the development of resistance to this agent in CMV strains capable of causing progressive disease .
	manualset3
168528	4	412959	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of ganciclovir in the treatment of cytomegalovirus ( CMV ) retinitis in patients with acquired immunodeficiency syndrome ( AIDS ) is limited by marrow toxicity and by the development of resistance to this agent in CMV strains capable of causing progressive disease .
	manualset3
168529	5	412959	7	NULL	NULL	NULL	NULL	acquired immunodeficiency syndrome ( AIDS )	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of ganciclovir in the treatment of cytomegalovirus ( CMV ) retinitis in patients with acquired immunodeficiency syndrome ( AIDS ) is limited by marrow toxicity and by the development of resistance to this agent in CMV strains capable of causing progressive disease .
	manualset3
168530	6	412959	7	NULL	NULL	0	NULL	marrow toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of ganciclovir in the treatment of cytomegalovirus ( CMV ) retinitis in patients with acquired immunodeficiency syndrome ( AIDS ) is limited by marrow toxicity and by the development of resistance to this agent in CMV strains capable of causing progressive disease .
	manualset3
168531	7	412959	7	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of ganciclovir in the treatment of cytomegalovirus ( CMV ) retinitis in patients with acquired immunodeficiency syndrome ( AIDS ) is limited by marrow toxicity and by the development of resistance to this agent in CMV strains capable of causing progressive disease .
	manualset3
168532	8	412959	7	NULL	NULL	0	NULL	resistance 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of ganciclovir in the treatment of cytomegalovirus ( CMV ) retinitis in patients with acquired immunodeficiency syndrome ( AIDS ) is limited by marrow toxicity and by the development of resistance to this agent in CMV strains capable of causing progressive disease .
	manualset3
168533	9	412959	7	NULL	NULL	0	NULL	agent	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of ganciclovir in the treatment of cytomegalovirus ( CMV ) retinitis in patients with acquired immunodeficiency syndrome ( AIDS ) is limited by marrow toxicity and by the development of resistance to this agent in CMV strains capable of causing progressive disease .
	manualset3
168534	10	412959	7	NULL	NULL	0	NULL	CMV strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of ganciclovir in the treatment of cytomegalovirus ( CMV ) retinitis in patients with acquired immunodeficiency syndrome ( AIDS ) is limited by marrow toxicity and by the development of resistance to this agent in CMV strains capable of causing progressive disease .
	manualset3
168535	11	412959	7	NULL	NULL	0	NULL	progressive disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of ganciclovir in the treatment of cytomegalovirus ( CMV ) retinitis in patients with acquired immunodeficiency syndrome ( AIDS ) is limited by marrow toxicity and by the development of resistance to this agent in CMV strains capable of causing progressive disease .
	manualset3
168536	1	412960	7	NULL	NULL	NULL	NULL	use of heterologous promoter	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of heterologous promoter and terminator sequences derived from the corn and soybean plastid genomes leads to simpler and predictable recombinant genome patterns , avoiding unwanted recombination products between introduced and resident tobacco sequences .
	manualset3
168537	2	412960	7	NULL	NULL	0	NULL	terminator sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of heterologous promoter and terminator sequences derived from the corn and soybean plastid genomes leads to simpler and predictable recombinant genome patterns , avoiding unwanted recombination products between introduced and resident tobacco sequences .
	manualset3
168538	3	412960	7	NULL	NULL	0	NULL	corn genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of heterologous promoter and terminator sequences derived from the corn and soybean plastid genomes leads to simpler and predictable recombinant genome patterns , avoiding unwanted recombination products between introduced and resident tobacco sequences .
	manualset3
168539	4	412960	7	NULL	NULL	0	NULL	soybean plastid genomes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of heterologous promoter and terminator sequences derived from the corn and soybean plastid genomes leads to simpler and predictable recombinant genome patterns , avoiding unwanted recombination products between introduced and resident tobacco sequences .
	manualset3
168540	5	412960	7	NULL	NULL	0	NULL	recombinant genome patterns	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of heterologous promoter and terminator sequences derived from the corn and soybean plastid genomes leads to simpler and predictable recombinant genome patterns , avoiding unwanted recombination products between introduced and resident tobacco sequences .
	manualset3
168541	6	412960	7	NULL	NULL	0	NULL	recombination products	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of heterologous promoter and terminator sequences derived from the corn and soybean plastid genomes leads to simpler and predictable recombinant genome patterns , avoiding unwanted recombination products between introduced and resident tobacco sequences .
	manualset3
168542	7	412960	7	NULL	NULL	0	NULL	introduced tobacco sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of heterologous promoter and terminator sequences derived from the corn and soybean plastid genomes leads to simpler and predictable recombinant genome patterns , avoiding unwanted recombination products between introduced and resident tobacco sequences .
	manualset3
168543	8	412960	7	NULL	NULL	0	NULL	resident tobacco sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of heterologous promoter and terminator sequences derived from the corn and soybean plastid genomes leads to simpler and predictable recombinant genome patterns , avoiding unwanted recombination products between introduced and resident tobacco sequences .
	manualset3
168544	1	412961	7	NULL	NULL	NULL	NULL	use of hypothermia	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of hypothermia and circulatory arrest in infancy has resulted in a considerably lower hospital mortality compared with cases operated on under conventional cardiopulmonary bypass .
	manualset3
168545	2	412961	7	NULL	NULL	0	NULL	circulatory arrest	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of hypothermia and circulatory arrest in infancy has resulted in a considerably lower hospital mortality compared with cases operated on under conventional cardiopulmonary bypass .
	manualset3
168546	3	412961	7	NULL	NULL	0	NULL	infancy	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of hypothermia and circulatory arrest in infancy has resulted in a considerably lower hospital mortality compared with cases operated on under conventional cardiopulmonary bypass .
	manualset3
168547	4	412961	7	NULL	NULL	0	NULL	 lower hospital mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of hypothermia and circulatory arrest in infancy has resulted in a considerably lower hospital mortality compared with cases operated on under conventional cardiopulmonary bypass .
	manualset3
168548	5	412961	7	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of hypothermia and circulatory arrest in infancy has resulted in a considerably lower hospital mortality compared with cases operated on under conventional cardiopulmonary bypass .
	manualset3
168549	6	412961	7	NULL	NULL	0	NULL	conventional cardiopulmonary bypass	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of hypothermia and circulatory arrest in infancy has resulted in a considerably lower hospital mortality compared with cases operated on under conventional cardiopulmonary bypass .
	manualset3
168550	1	412962	7	NULL	NULL	NULL	NULL	use of in vivo IOS	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of in vivo IOS to record spatial maps started in the mid 1980 's with the observation of optical maps of whisker barrels in the rat and the orientation columns in the cat visual cortex ( 1 ) .
	manualset3
168551	2	412962	7	NULL	NULL	0	NULL	spatial maps	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of in vivo IOS to record spatial maps started in the mid 1980 's with the observation of optical maps of whisker barrels in the rat and the orientation columns in the cat visual cortex ( 1 ) .
	manualset3
168552	3	412962	7	NULL	NULL	0	NULL	mid 1980 's	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of in vivo IOS to record spatial maps started in the mid 1980 's with the observation of optical maps of whisker barrels in the rat and the orientation columns in the cat visual cortex ( 1 ) .
	manualset3
168553	4	412962	7	NULL	NULL	0	NULL	observation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of in vivo IOS to record spatial maps started in the mid 1980 's with the observation of optical maps of whisker barrels in the rat and the orientation columns in the cat visual cortex ( 1 ) .
	manualset3
168554	5	412962	7	NULL	NULL	0	NULL	optical maps	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of in vivo IOS to record spatial maps started in the mid 1980 's with the observation of optical maps of whisker barrels in the rat and the orientation columns in the cat visual cortex ( 1 ) .
	manualset3
168555	6	412962	7	NULL	NULL	NULL	NULL	whisker barrels	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of in vivo IOS to record spatial maps started in the mid 1980 's with the observation of optical maps of whisker barrels in the rat and the orientation columns in the cat visual cortex ( 1 ) .
	manualset3
168556	7	412962	7	NULL	NULL	0	NULL	 rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of in vivo IOS to record spatial maps started in the mid 1980 's with the observation of optical maps of whisker barrels in the rat and the orientation columns in the cat visual cortex ( 1 ) .
	manualset3
168557	8	412962	7	NULL	NULL	0	NULL	orientation columns	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of in vivo IOS to record spatial maps started in the mid 1980 's with the observation of optical maps of whisker barrels in the rat and the orientation columns in the cat visual cortex ( 1 ) .
	manualset3
168558	9	412962	7	NULL	NULL	0	NULL	cat visual cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of in vivo IOS to record spatial maps started in the mid 1980 's with the observation of optical maps of whisker barrels in the rat and the orientation columns in the cat visual cortex ( 1 ) .
	manualset3
168559	2	412963	7	NULL	NULL	NULL	NULL	use of in vivo direct drug application	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of in vivo direct drug application to assess neural regulation of muscle properties .
	manualset3
168560	3	412963	7	NULL	NULL	NULL	NULL	neural regulation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of in vivo direct drug application to assess neural regulation of muscle properties .
	manualset3
168561	4	412963	7	NULL	NULL	0	NULL	muscle properties	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of in vivo direct drug application to assess neural regulation of muscle properties .
	manualset3
168564	2	412964	7	NULL	NULL	NULL	NULL	 use of integrins	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of integrins in drug targeting and integrins as targets for drug delivery by using the RGD as a template structure will also be discussed .
	manualset3
168565	3	412964	7	NULL	NULL	0	NULL	drug targeting	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of integrins in drug targeting and integrins as targets for drug delivery by using the RGD as a template structure will also be discussed .
	manualset3
168566	4	412964	7	NULL	NULL	0	NULL	integrins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of integrins in drug targeting and integrins as targets for drug delivery by using the RGD as a template structure will also be discussed .
	manualset3
168567	5	412964	7	NULL	NULL	0	NULL	 targets	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of integrins in drug targeting and integrins as targets for drug delivery by using the RGD as a template structure will also be discussed .
	manualset3
168568	6	412964	7	NULL	NULL	0	NULL	drug delivery	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of integrins in drug targeting and integrins as targets for drug delivery by using the RGD as a template structure will also be discussed .
	manualset3
168569	7	412964	7	NULL	NULL	0	NULL	RGD 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of integrins in drug targeting and integrins as targets for drug delivery by using the RGD as a template structure will also be discussed .
	manualset3
168570	8	412964	7	NULL	NULL	0	NULL	template structure	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of integrins in drug targeting and integrins as targets for drug delivery by using the RGD as a template structure will also be discussed .
	manualset3
168572	2	412965	7	NULL	NULL	NULL	NULL	use of marker proteins	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of marker proteins promises to promote our understanding of the mechanism of implantation while providing clues into the causes of some types of infertility .
	manualset3
168573	3	412965	7	NULL	NULL	0	NULL	understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of marker proteins promises to promote our understanding of the mechanism of implantation while providing clues into the causes of some types of infertility .
	manualset3
168574	4	412965	7	NULL	NULL	0	NULL	mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of marker proteins promises to promote our understanding of the mechanism of implantation while providing clues into the causes of some types of infertility .
	manualset3
168575	5	412965	7	NULL	NULL	0	NULL	implantation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of marker proteins promises to promote our understanding of the mechanism of implantation while providing clues into the causes of some types of infertility .
	manualset3
168576	6	412965	7	NULL	NULL	0	NULL	causes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of marker proteins promises to promote our understanding of the mechanism of implantation while providing clues into the causes of some types of infertility .
	manualset3
168577	7	412965	7	NULL	NULL	0	NULL	types of infertility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of marker proteins promises to promote our understanding of the mechanism of implantation while providing clues into the causes of some types of infertility .
	manualset3
168579	2	412966	7	NULL	NULL	NULL	NULL	use of naloxone	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of naloxone in small doses in complex therapy of postabstinent heroin syndrome : enkephalinase mechanisms .
	manualset3
168580	3	412966	7	NULL	NULL	0	NULL	small doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of naloxone in small doses in complex therapy of postabstinent heroin syndrome : enkephalinase mechanisms .
	manualset3
168581	4	412966	7	NULL	NULL	0	NULL	complex therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of naloxone in small doses in complex therapy of postabstinent heroin syndrome : enkephalinase mechanisms .
	manualset3
168582	5	412966	7	NULL	NULL	0	NULL	postabstinent heroin syndrome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of naloxone in small doses in complex therapy of postabstinent heroin syndrome : enkephalinase mechanisms .
	manualset3
168583	6	412966	7	NULL	NULL	NULL	NULL	enkephalinase mechanisms	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of naloxone in small doses in complex therapy of postabstinent heroin syndrome : enkephalinase mechanisms .
	manualset3
168585	2	412967	7	NULL	NULL	NULL	NULL	use of noise bursts	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of noise bursts to produce the nonG noise instead of impacts also reduced the amount of trauma .
	manualset3
168586	3	412967	7	NULL	NULL	0	NULL	nonG noise	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of noise bursts to produce the nonG noise instead of impacts also reduced the amount of trauma .
	manualset3
168587	4	412967	7	NULL	NULL	0	NULL	impacts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of noise bursts to produce the nonG noise instead of impacts also reduced the amount of trauma .
	manualset3
168588	5	412967	7	NULL	NULL	0	NULL	amount	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of noise bursts to produce the nonG noise instead of impacts also reduced the amount of trauma .
	manualset3
168589	6	412967	7	NULL	NULL	0	NULL	trauma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of noise bursts to produce the nonG noise instead of impacts also reduced the amount of trauma .
	manualset3
168590	1	412968	7	NULL	NULL	0	NULL	Actinobacillus actinomycetemcomitans leukotoxin ( Ltx )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Actinobacillus actinomycetemcomitans leukotoxin ( Ltx ) is a member of the repeats-in-toxin ( RTX ) family of pore-forming toxins and kills human immune cells .
	manualset3
168591	2	412968	7	NULL	NULL	0	NULL	member	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Actinobacillus actinomycetemcomitans leukotoxin ( Ltx ) is a member of the repeats-in-toxin ( RTX ) family of pore-forming toxins and kills human immune cells .
	manualset3
168592	3	412968	7	NULL	NULL	0	NULL	repeats-in-toxin ( RTX ) family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Actinobacillus actinomycetemcomitans leukotoxin ( Ltx ) is a member of the repeats-in-toxin ( RTX ) family of pore-forming toxins and kills human immune cells .
	manualset3
168593	4	412968	7	NULL	NULL	NULL	NULL	pore-forming toxins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Actinobacillus actinomycetemcomitans leukotoxin ( Ltx ) is a member of the repeats-in-toxin ( RTX ) family of pore-forming toxins and kills human immune cells .
	manualset3
168594	5	412968	7	NULL	NULL	0	NULL	human immune cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Actinobacillus actinomycetemcomitans leukotoxin ( Ltx ) is a member of the repeats-in-toxin ( RTX ) family of pore-forming toxins and kills human immune cells .
	manualset3
168596	2	412969	7	NULL	NULL	NULL	NULL	use of non-steroidal anti-inflammatory agents	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of non-steroidal anti-inflammatory agents in these conditions remains controversial ; their possible beneficial effects are believed to be due to inhibition of TXA2 synthesis whereas their failure to be effective may be a consequence of concomitant inhibition of PGI2 production .
	manualset3
168597	3	412969	7	NULL	NULL	0	NULL	conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of non-steroidal anti-inflammatory agents in these conditions remains controversial ; their possible beneficial effects are believed to be due to inhibition of TXA2 synthesis whereas their failure to be effective may be a consequence of concomitant inhibition of PGI2 production .
	manualset3
168598	4	412969	7	NULL	NULL	0	NULL	beneficial effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of non-steroidal anti-inflammatory agents in these conditions remains controversial ; their possible beneficial effects are believed to be due to inhibition of TXA2 synthesis whereas their failure to be effective may be a consequence of concomitant inhibition of PGI2 production .
	manualset3
168599	5	412969	7	NULL	NULL	0	NULL	inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of non-steroidal anti-inflammatory agents in these conditions remains controversial ; their possible beneficial effects are believed to be due to inhibition of TXA2 synthesis whereas their failure to be effective may be a consequence of concomitant inhibition of PGI2 production .
	manualset3
168600	6	412969	7	NULL	NULL	0	NULL	 TXA2 synthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of non-steroidal anti-inflammatory agents in these conditions remains controversial ; their possible beneficial effects are believed to be due to inhibition of TXA2 synthesis whereas their failure to be effective may be a consequence of concomitant inhibition of PGI2 production .
	manualset3
168601	7	412969	7	NULL	NULL	0	NULL	failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of non-steroidal anti-inflammatory agents in these conditions remains controversial ; their possible beneficial effects are believed to be due to inhibition of TXA2 synthesis whereas their failure to be effective may be a consequence of concomitant inhibition of PGI2 production .
	manualset3
168602	8	412969	7	NULL	NULL	0	NULL	consequence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of non-steroidal anti-inflammatory agents in these conditions remains controversial ; their possible beneficial effects are believed to be due to inhibition of TXA2 synthesis whereas their failure to be effective may be a consequence of concomitant inhibition of PGI2 production .
	manualset3
168603	9	412969	7	NULL	NULL	0	NULL	concomitant inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of non-steroidal anti-inflammatory agents in these conditions remains controversial ; their possible beneficial effects are believed to be due to inhibition of TXA2 synthesis whereas their failure to be effective may be a consequence of concomitant inhibition of PGI2 production .
	manualset3
168604	10	412969	7	NULL	NULL	0	NULL	PGI2 production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of non-steroidal anti-inflammatory agents in these conditions remains controversial ; their possible beneficial effects are believed to be due to inhibition of TXA2 synthesis whereas their failure to be effective may be a consequence of concomitant inhibition of PGI2 production .
	manualset3
168606	2	412970	7	NULL	NULL	NULL	NULL	use of numerical methods	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of numerical methods for qualitative and quantitative evaluation of the degree of pollution .
	manualset3
168607	3	412970	7	NULL	NULL	0	NULL	qualitative evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of numerical methods for qualitative and quantitative evaluation of the degree of pollution .
	manualset3
168608	4	412970	7	NULL	NULL	0	NULL	quantitative evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of numerical methods for qualitative and quantitative evaluation of the degree of pollution .
	manualset3
168609	5	412970	7	NULL	NULL	0	NULL	degree	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of numerical methods for qualitative and quantitative evaluation of the degree of pollution .
	manualset3
168610	6	412970	7	NULL	NULL	0	NULL	pollution	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of numerical methods for qualitative and quantitative evaluation of the degree of pollution .
	manualset3
168612	2	412971	7	NULL	NULL	NULL	NULL	use of uoncolytic vaccinia viruses	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of oncolytic vaccinia viruses in the treatment of cancer : a new role for an old ally ?
	manualset3
168613	3	412971	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of oncolytic vaccinia viruses in the treatment of cancer : a new role for an old ally ?
	manualset3
168614	4	412971	7	NULL	NULL	0	NULL	cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of oncolytic vaccinia viruses in the treatment of cancer : a new role for an old ally ?
	manualset3
168615	5	412971	7	NULL	NULL	0	NULL	a new role for an old ally ?	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of oncolytic vaccinia viruses in the treatment of cancer : a new role for an old ally ?
	manualset3
168617	2	412972	7	NULL	NULL	NULL	NULL	use of peripheral DXA	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of peripheral DXA is growing in primary care and guidance on its use has recently been published by the National Osteoporosis Society ( NOS ) , recommending a triage approach using thresholds specific to each type of peripheral device .
	manualset3
168618	3	412972	7	NULL	NULL	0	NULL	primary care 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of peripheral DXA is growing in primary care and guidance on its use has recently been published by the National Osteoporosis Society ( NOS ) , recommending a triage approach using thresholds specific to each type of peripheral device .
	manualset3
168619	4	412972	7	NULL	NULL	0	NULL	guidance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of peripheral DXA is growing in primary care and guidance on its use has recently been published by the National Osteoporosis Society ( NOS ) , recommending a triage approach using thresholds specific to each type of peripheral device .
	manualset3
168620	5	412972	7	NULL	NULL	0	NULL	National Osteoporosis Society ( NOS ) 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of peripheral DXA is growing in primary care and guidance on its use has recently been published by the National Osteoporosis Society ( NOS ) , recommending a triage approach using thresholds specific to each type of peripheral device .
	manualset3
168621	6	412972	7	NULL	NULL	NULL	NULL	triage approach 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of peripheral DXA is growing in primary care and guidance on its use has recently been published by the National Osteoporosis Society ( NOS ) , recommending a triage approach using thresholds specific to each type of peripheral device .
	manualset3
168622	7	412972	7	NULL	NULL	0	NULL	thresholds 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of peripheral DXA is growing in primary care and guidance on its use has recently been published by the National Osteoporosis Society ( NOS ) , recommending a triage approach using thresholds specific to each type of peripheral device .
	manualset3
168623	8	412972	7	NULL	NULL	NULL	NULL	type of peripheral device	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of peripheral DXA is growing in primary care and guidance on its use has recently been published by the National Osteoporosis Society ( NOS ) , recommending a triage approach using thresholds specific to each type of peripheral device .
	manualset3
168625	2	412973	7	NULL	NULL	NULL	NULL	antiretroviral regimens	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of previously successful antiretroviral regimens in mother-to-child transmission ( MTCT ) prevention will be increasingly challenged by the rising prevalence of multidrug-resistant ( MDR ) HIV .
	manualset3
168626	3	412973	7	NULL	NULL	0	NULL	mother-to-child transmission ( MTCT ) prevention	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of previously successful antiretroviral regimens in mother-to-child transmission ( MTCT ) prevention will be increasingly challenged by the rising prevalence of multidrug-resistant ( MDR ) HIV .
	manualset3
168627	4	412973	7	NULL	NULL	0	NULL	prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of previously successful antiretroviral regimens in mother-to-child transmission ( MTCT ) prevention will be increasingly challenged by the rising prevalence of multidrug-resistant ( MDR ) HIV .
	manualset3
168628	5	412973	7	NULL	NULL	NULL	NULL	multidrug-resistant ( MDR ) HIV	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of previously successful antiretroviral regimens in mother-to-child transmission ( MTCT ) prevention will be increasingly challenged by the rising prevalence of multidrug-resistant ( MDR ) HIV .
	manualset3
168631	2	412974	7	NULL	NULL	NULL	NULL	 use of teleradiology	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of teleradiology has grown tremendously during the past few years .
	manualset3
168632	3	412974	7	NULL	NULL	0	NULL	past few years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of teleradiology has grown tremendously during the past few years .
	manualset3
168634	2	412975	7	NULL	NULL	NULL	NULL	use of F9 cell line	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of the F9 cell line in in vitro teratogenicity testing shows promise , but further work is necessary before its potential can be fully evaluated .
	manualset3
168635	3	412975	7	NULL	NULL	0	NULL	in vitro teratogenicity testing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of the F9 cell line in in vitro teratogenicity testing shows promise , but further work is necessary before its potential can be fully evaluated .
	manualset3
168636	4	412975	7	NULL	NULL	0	NULL	work 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of the F9 cell line in in vitro teratogenicity testing shows promise , but further work is necessary before its potential can be fully evaluated .
	manualset3
168637	5	412975	7	NULL	NULL	NULL	NULL	potential	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of the F9 cell line in in vitro teratogenicity testing shows promise , but further work is necessary before its potential can be fully evaluated .
	manualset3
168639	2	412976	7	NULL	NULL	NULL	NULL	use of dietary supplement SeleniumEC 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of the dietary supplement SeleniumEC resulted in the normalization of markers of the lipid peroxidation and the antioxidant system during complex diet therapy of patients with ischemic heart diseases .
	manualset3
168640	3	412976	7	NULL	NULL	0	NULL	normalization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of the dietary supplement SeleniumEC resulted in the normalization of markers of the lipid peroxidation and the antioxidant system during complex diet therapy of patients with ischemic heart diseases .
	manualset3
168641	4	412976	7	NULL	NULL	0	NULL	 markers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of the dietary supplement SeleniumEC resulted in the normalization of markers of the lipid peroxidation and the antioxidant system during complex diet therapy of patients with ischemic heart diseases .
	manualset3
168642	5	412976	7	NULL	NULL	0	NULL	lipid peroxidation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of the dietary supplement SeleniumEC resulted in the normalization of markers of the lipid peroxidation and the antioxidant system during complex diet therapy of patients with ischemic heart diseases .
	manualset3
168643	6	412976	7	NULL	NULL	0	NULL	antioxidant system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of the dietary supplement SeleniumEC resulted in the normalization of markers of the lipid peroxidation and the antioxidant system during complex diet therapy of patients with ischemic heart diseases .
	manualset3
168644	7	412976	7	NULL	NULL	0	NULL	complex diet therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of the dietary supplement SeleniumEC resulted in the normalization of markers of the lipid peroxidation and the antioxidant system during complex diet therapy of patients with ischemic heart diseases .
	manualset3
168645	8	412976	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of the dietary supplement SeleniumEC resulted in the normalization of markers of the lipid peroxidation and the antioxidant system during complex diet therapy of patients with ischemic heart diseases .
	manualset3
168646	9	412976	7	NULL	NULL	0	NULL	ischemic heart diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of the dietary supplement SeleniumEC resulted in the normalization of markers of the lipid peroxidation and the antioxidant system during complex diet therapy of patients with ischemic heart diseases .
	manualset3
168647	1	412977	7	NULL	NULL	0	NULL	Action	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Action of biogenic amines injected intracerebrally on duration of hexobarbital-induced sleep in rats .
	manualset3
168648	2	412977	7	NULL	NULL	0	NULL	biogenic amines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Action of biogenic amines injected intracerebrally on duration of hexobarbital-induced sleep in rats .
	manualset3
168649	3	412977	7	NULL	NULL	0	NULL	duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Action of biogenic amines injected intracerebrally on duration of hexobarbital-induced sleep in rats .
	manualset3
168650	4	412977	7	NULL	NULL	0	NULL	hexobarbital-induced sleep	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Action of biogenic amines injected intracerebrally on duration of hexobarbital-induced sleep in rats .
	manualset3
168651	5	412977	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Action of biogenic amines injected intracerebrally on duration of hexobarbital-induced sleep in rats .
	manualset3
168653	2	412978	7	NULL	NULL	NULL	NULL	use of the method 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of the method for treatment of 4 patients with tumors of the vertebrae has revealed a number of problems requiring a somewhat different approach both to the performance of the operation and to the following fixation of the backbone .
	manualset3
168654	3	412978	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of the method for treatment of 4 patients with tumors of the vertebrae has revealed a number of problems requiring a somewhat different approach both to the performance of the operation and to the following fixation of the backbone .
	manualset3
168655	4	412978	7	NULL	NULL	0	NULL	4 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of the method for treatment of 4 patients with tumors of the vertebrae has revealed a number of problems requiring a somewhat different approach both to the performance of the operation and to the following fixation of the backbone .
	manualset3
168656	5	412978	7	NULL	NULL	0	NULL	tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of the method for treatment of 4 patients with tumors of the vertebrae has revealed a number of problems requiring a somewhat different approach both to the performance of the operation and to the following fixation of the backbone .
	manualset3
168657	6	412978	7	NULL	NULL	NULL	NULL	vertebrae	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of the method for treatment of 4 patients with tumors of the vertebrae has revealed a number of problems requiring a somewhat different approach both to the performance of the operation and to the following fixation of the backbone .
	manualset3
168658	7	412978	7	NULL	NULL	NULL	NULL	 number of problems	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of the method for treatment of 4 patients with tumors of the vertebrae has revealed a number of problems requiring a somewhat different approach both to the performance of the operation and to the following fixation of the backbone .
	manualset3
168660	9	412978	7	NULL	NULL	NULL	NULL	approach	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of the method for treatment of 4 patients with tumors of the vertebrae has revealed a number of problems requiring a somewhat different approach both to the performance of the operation and to the following fixation of the backbone .
	manualset3
168661	10	412978	7	NULL	NULL	NULL	NULL	performance of the operation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of the method for treatment of 4 patients with tumors of the vertebrae has revealed a number of problems requiring a somewhat different approach both to the performance of the operation and to the following fixation of the backbone .
	manualset3
168663	12	412978	7	NULL	NULL	0	NULL	fixation of the backbone	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of the method for treatment of 4 patients with tumors of the vertebrae has revealed a number of problems requiring a somewhat different approach both to the performance of the operation and to the following fixation of the backbone .
	manualset3
168665	2	412979	7	NULL	NULL	NULL	NULL	use of the software package	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of the software package EndNote 4 for Windows is described , and we want to report about our own experiences with the new version of this database manager .
	manualset3
168666	3	412979	7	NULL	NULL	0	NULL	EndNote 4	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of the software package EndNote 4 for Windows is described , and we want to report about our own experiences with the new version of this database manager .
	manualset3
168667	4	412979	7	NULL	NULL	0	NULL	Windows	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of the software package EndNote 4 for Windows is described , and we want to report about our own experiences with the new version of this database manager .
	manualset3
168668	5	412979	7	NULL	NULL	0	NULL	experiences	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of the software package EndNote 4 for Windows is described , and we want to report about our own experiences with the new version of this database manager .
	manualset3
168669	6	412979	7	NULL	NULL	0	NULL	new version	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of the software package EndNote 4 for Windows is described , and we want to report about our own experiences with the new version of this database manager .
	manualset3
168670	7	412979	7	NULL	NULL	0	NULL	database manager	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of the software package EndNote 4 for Windows is described , and we want to report about our own experiences with the new version of this database manager .
	manualset3
168672	1	412980	7	NULL	NULL	NULL	NULL	use of therapeutic drug monitoring ( TDM )	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of therapeutic drug monitoring ( TDM ) in the treatment of HIV-infection is gaining momentum in resource-rich countries .
	manualset3
168673	3	412980	7	NULL	NULL	0	NULL	 treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of therapeutic drug monitoring ( TDM ) in the treatment of HIV-infection is gaining momentum in resource-rich countries .
	manualset3
168674	4	412980	7	NULL	NULL	0	NULL	HIV-infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of therapeutic drug monitoring ( TDM ) in the treatment of HIV-infection is gaining momentum in resource-rich countries .
	manualset3
168675	5	412980	7	NULL	NULL	0	NULL	resource-rich countries	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of therapeutic drug monitoring ( TDM ) in the treatment of HIV-infection is gaining momentum in resource-rich countries .
	manualset3
168677	1	412981	7	NULL	NULL	NULL	NULL	use of thermal infrared imaging	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of thermal infrared imaging to assess the efficacy of a therapeutic exercise program in individuals with diabetes .
	manualset3
168678	3	412981	7	NULL	NULL	0	NULL	efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of thermal infrared imaging to assess the efficacy of a therapeutic exercise program in individuals with diabetes .
	manualset3
168679	4	412981	7	NULL	NULL	0	NULL	therapeutic exercise program	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of thermal infrared imaging to assess the efficacy of a therapeutic exercise program in individuals with diabetes .
	manualset3
168680	5	412981	7	NULL	NULL	0	NULL	individuals	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of thermal infrared imaging to assess the efficacy of a therapeutic exercise program in individuals with diabetes .
	manualset3
168681	6	412981	7	NULL	NULL	NULL	NULL	 diabetes 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of thermal infrared imaging to assess the efficacy of a therapeutic exercise program in individuals with diabetes .
	manualset3
168684	1	412982	7	NULL	NULL	NULL	NULL	use of transfusion regime	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of this transfusion regime for hemodynamic re-equilibration in upper gastro-intestinal hemorrhage due to ulcer , in cases in which hemostasis can be obtained with certainty by emergency surgery , allows transfusion of stored blood and colloid solutions to be avoided and emergency surgery to be safely undertaken at the earliest moment .
	manualset3
168685	3	412982	7	NULL	NULL	0	NULL	hemodynamic re-equilibration 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of this transfusion regime for hemodynamic re-equilibration in upper gastro-intestinal hemorrhage due to ulcer , in cases in which hemostasis can be obtained with certainty by emergency surgery , allows transfusion of stored blood and colloid solutions to be avoided and emergency surgery to be safely undertaken at the earliest moment .
	manualset3
168686	4	412982	7	NULL	NULL	0	NULL	upper gastro-intestinal hemorrhage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of this transfusion regime for hemodynamic re-equilibration in upper gastro-intestinal hemorrhage due to ulcer , in cases in which hemostasis can be obtained with certainty by emergency surgery , allows transfusion of stored blood and colloid solutions to be avoided and emergency surgery to be safely undertaken at the earliest moment .
	manualset3
168687	5	412982	7	NULL	NULL	0	NULL	 ulcer 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of this transfusion regime for hemodynamic re-equilibration in upper gastro-intestinal hemorrhage due to ulcer , in cases in which hemostasis can be obtained with certainty by emergency surgery , allows transfusion of stored blood and colloid solutions to be avoided and emergency surgery to be safely undertaken at the earliest moment .
	manualset3
168688	6	412982	7	NULL	NULL	0	NULL	cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of this transfusion regime for hemodynamic re-equilibration in upper gastro-intestinal hemorrhage due to ulcer , in cases in which hemostasis can be obtained with certainty by emergency surgery , allows transfusion of stored blood and colloid solutions to be avoided and emergency surgery to be safely undertaken at the earliest moment .
	manualset3
168689	7	412982	7	NULL	NULL	0	NULL	hemostasis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of this transfusion regime for hemodynamic re-equilibration in upper gastro-intestinal hemorrhage due to ulcer , in cases in which hemostasis can be obtained with certainty by emergency surgery , allows transfusion of stored blood and colloid solutions to be avoided and emergency surgery to be safely undertaken at the earliest moment .
	manualset3
168690	8	412982	7	NULL	NULL	0	NULL	emergency surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of this transfusion regime for hemodynamic re-equilibration in upper gastro-intestinal hemorrhage due to ulcer , in cases in which hemostasis can be obtained with certainty by emergency surgery , allows transfusion of stored blood and colloid solutions to be avoided and emergency surgery to be safely undertaken at the earliest moment .
	manualset3
168691	9	412982	7	NULL	NULL	0	NULL	transfusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of this transfusion regime for hemodynamic re-equilibration in upper gastro-intestinal hemorrhage due to ulcer , in cases in which hemostasis can be obtained with certainty by emergency surgery , allows transfusion of stored blood and colloid solutions to be avoided and emergency surgery to be safely undertaken at the earliest moment .
	manualset3
168692	10	412982	7	NULL	NULL	0	NULL	stored blood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of this transfusion regime for hemodynamic re-equilibration in upper gastro-intestinal hemorrhage due to ulcer , in cases in which hemostasis can be obtained with certainty by emergency surgery , allows transfusion of stored blood and colloid solutions to be avoided and emergency surgery to be safely undertaken at the earliest moment .
	manualset3
168693	11	412982	7	NULL	NULL	0	NULL	colloid solutions 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of this transfusion regime for hemodynamic re-equilibration in upper gastro-intestinal hemorrhage due to ulcer , in cases in which hemostasis can be obtained with certainty by emergency surgery , allows transfusion of stored blood and colloid solutions to be avoided and emergency surgery to be safely undertaken at the earliest moment .
	manualset3
168694	12	412982	7	NULL	NULL	0	NULL	emergency surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of this transfusion regime for hemodynamic re-equilibration in upper gastro-intestinal hemorrhage due to ulcer , in cases in which hemostasis can be obtained with certainty by emergency surgery , allows transfusion of stored blood and colloid solutions to be avoided and emergency surgery to be safely undertaken at the earliest moment .
	manualset3
168695	13	412982	7	NULL	NULL	0	NULL	earliest moment	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of this transfusion regime for hemodynamic re-equilibration in upper gastro-intestinal hemorrhage due to ulcer , in cases in which hemostasis can be obtained with certainty by emergency surgery , allows transfusion of stored blood and colloid solutions to be avoided and emergency surgery to be safely undertaken at the earliest moment .
	manualset3
168697	1	412983	7	NULL	NULL	NULL	NULL	use of ultrasound 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of ultrasound to enhance the diagnostic utility of the equivocal liver scintigraph .
	manualset3
168698	3	412983	7	NULL	NULL	0	NULL	diagnostic utility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of ultrasound to enhance the diagnostic utility of the equivocal liver scintigraph .
	manualset3
168699	4	412983	7	NULL	NULL	0	NULL	equivocal liver scintigraph	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of ultrasound to enhance the diagnostic utility of the equivocal liver scintigraph .
	manualset3
168701	2	412984	7	NULL	NULL	NULL	NULL	use of written materials	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of written materials and early antenatal education may improve retention of information and maternal satisfaction .
	manualset3
168702	3	412984	7	NULL	NULL	0	NULL	early antenatal education	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of written materials and early antenatal education may improve retention of information and maternal satisfaction .
	manualset3
168703	4	412984	7	NULL	NULL	0	NULL	retention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of written materials and early antenatal education may improve retention of information and maternal satisfaction .
	manualset3
168704	5	412984	7	NULL	NULL	0	NULL	information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of written materials and early antenatal education may improve retention of information and maternal satisfaction .
	manualset3
168705	6	412984	7	NULL	NULL	NULL	NULL	maternal satisfaction	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of written materials and early antenatal education may improve retention of information and maternal satisfaction .
	manualset3
168706	1	412985	7	NULL	NULL	NULL	NULL	usefulness 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The usefulness of determining the renal handling of endogenous lithium as a marker of proximal tubular sodium reabsorption was assessed in streptozotocin induced diabetes mellitus in the Sprague-Dawley rat .
	manualset3
168707	2	412985	7	NULL	NULL	0	NULL	renal handling	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The usefulness of determining the renal handling of endogenous lithium as a marker of proximal tubular sodium reabsorption was assessed in streptozotocin induced diabetes mellitus in the Sprague-Dawley rat .
	manualset3
168708	3	412985	7	NULL	NULL	0	NULL	endogenous lithium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The usefulness of determining the renal handling of endogenous lithium as a marker of proximal tubular sodium reabsorption was assessed in streptozotocin induced diabetes mellitus in the Sprague-Dawley rat .
	manualset3
168709	4	412985	7	NULL	NULL	0	NULL	marker	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The usefulness of determining the renal handling of endogenous lithium as a marker of proximal tubular sodium reabsorption was assessed in streptozotocin induced diabetes mellitus in the Sprague-Dawley rat .
	manualset3
168710	5	412985	7	NULL	NULL	0	NULL	proximal tubular sodium reabsorption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The usefulness of determining the renal handling of endogenous lithium as a marker of proximal tubular sodium reabsorption was assessed in streptozotocin induced diabetes mellitus in the Sprague-Dawley rat .
	manualset3
168711	6	412985	7	NULL	NULL	0	NULL	streptozotocin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The usefulness of determining the renal handling of endogenous lithium as a marker of proximal tubular sodium reabsorption was assessed in streptozotocin induced diabetes mellitus in the Sprague-Dawley rat .
	manualset3
168712	7	412985	7	NULL	NULL	0	NULL	diabetes mellitus 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The usefulness of determining the renal handling of endogenous lithium as a marker of proximal tubular sodium reabsorption was assessed in streptozotocin induced diabetes mellitus in the Sprague-Dawley rat .
	manualset3
168713	8	412985	7	NULL	NULL	0	NULL	Sprague-Dawley rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The usefulness of determining the renal handling of endogenous lithium as a marker of proximal tubular sodium reabsorption was assessed in streptozotocin induced diabetes mellitus in the Sprague-Dawley rat .
	manualset3
168714	1	412986	7	NULL	NULL	0	NULL	Action	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Action of progesterone and of 17-beta-estradiol in various combinations ) .
	manualset3
168715	2	412986	7	NULL	NULL	0	NULL	progesterone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Action of progesterone and of 17-beta-estradiol in various combinations ) .
	manualset3
168716	3	412986	7	NULL	NULL	0	NULL	17-beta-estradiol 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Action of progesterone and of 17-beta-estradiol in various combinations ) .
	manualset3
168717	4	412986	7	NULL	NULL	0	NULL	combinations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Action of progesterone and of 17-beta-estradiol in various combinations ) .
	manualset3
168718	1	412987	7	NULL	NULL	0	NULL	usefulness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The usefulness of the method in drug design has been demonstrated by the fact that inhibitor 5 , designed by us was found to bind more tightly than MTX , by as much 7.5 kcal/mole and is a worthy candidate for further pharmacological investigations .
	manualset3
168719	2	412987	7	NULL	NULL	0	NULL	 method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The usefulness of the method in drug design has been demonstrated by the fact that inhibitor 5 , designed by us was found to bind more tightly than MTX , by as much 7.5 kcal/mole and is a worthy candidate for further pharmacological investigations .
	manualset3
168720	3	412987	7	NULL	NULL	0	NULL	drug design	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The usefulness of the method in drug design has been demonstrated by the fact that inhibitor 5 , designed by us was found to bind more tightly than MTX , by as much 7.5 kcal/mole and is a worthy candidate for further pharmacological investigations .
	manualset3
168721	4	412987	7	NULL	NULL	0	NULL	inhibitor 5	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The usefulness of the method in drug design has been demonstrated by the fact that inhibitor 5 , designed by us was found to bind more tightly than MTX , by as much 7.5 kcal/mole and is a worthy candidate for further pharmacological investigations .
	manualset3
168722	5	412987	7	NULL	NULL	0	NULL	MTX	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The usefulness of the method in drug design has been demonstrated by the fact that inhibitor 5 , designed by us was found to bind more tightly than MTX , by as much 7.5 kcal/mole and is a worthy candidate for further pharmacological investigations .
	manualset3
168723	6	412987	7	NULL	NULL	0	NULL	7.5 kcal/mole	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The usefulness of the method in drug design has been demonstrated by the fact that inhibitor 5 , designed by us was found to bind more tightly than MTX , by as much 7.5 kcal/mole and is a worthy candidate for further pharmacological investigations .
	manualset3
168724	7	412987	7	NULL	NULL	0	NULL	candidate	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The usefulness of the method in drug design has been demonstrated by the fact that inhibitor 5 , designed by us was found to bind more tightly than MTX , by as much 7.5 kcal/mole and is a worthy candidate for further pharmacological investigations .
	manualset3
168725	8	412987	7	NULL	NULL	0	NULL	pharmacological investigations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The usefulness of the method in drug design has been demonstrated by the fact that inhibitor 5 , designed by us was found to bind more tightly than MTX , by as much 7.5 kcal/mole and is a worthy candidate for further pharmacological investigations .
	manualset3
168726	1	412988	7	NULL	NULL	0	NULL	 usual site	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The usual site of occurrence is the face , including the nose and eyelid .
	manualset3
168727	2	412988	7	NULL	NULL	0	NULL	face	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The usual site of occurrence is the face , including the nose and eyelid .
	manualset3
168728	3	412988	7	NULL	NULL	0	NULL	nose	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The usual site of occurrence is the face , including the nose and eyelid .
	manualset3
168729	4	412988	7	NULL	NULL	0	NULL	eyelid	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The usual site of occurrence is the face , including the nose and eyelid .
	manualset3
170375	5	412988	7	NULL	NULL	0	NULL	occurence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The usual site of occurrence is the face , including the nose and eyelid .
	manualset3
168730	1	412989	7	NULL	NULL	0	NULL	 utility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The utility of the approach was illustrated by investigating the metabolism of the drugs diclofenac ( DCF ) , troglitazone ( TGZ ) , and raloxifene , for which we observed known metabolic oxidation and bioconjugation pathways and turnover rates .
	manualset3
168731	2	412989	7	NULL	NULL	0	NULL	approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The utility of the approach was illustrated by investigating the metabolism of the drugs diclofenac ( DCF ) , troglitazone ( TGZ ) , and raloxifene , for which we observed known metabolic oxidation and bioconjugation pathways and turnover rates .
	manualset3
168732	3	412989	7	NULL	NULL	NULL	NULL	metabolism	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The utility of the approach was illustrated by investigating the metabolism of the drugs diclofenac ( DCF ) , troglitazone ( TGZ ) , and raloxifene , for which we observed known metabolic oxidation and bioconjugation pathways and turnover rates .
	manualset3
168733	4	412989	7	NULL	NULL	0	NULL	drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The utility of the approach was illustrated by investigating the metabolism of the drugs diclofenac ( DCF ) , troglitazone ( TGZ ) , and raloxifene , for which we observed known metabolic oxidation and bioconjugation pathways and turnover rates .
	manualset3
168734	5	412989	7	NULL	NULL	0	NULL	diclofenac ( DCF )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The utility of the approach was illustrated by investigating the metabolism of the drugs diclofenac ( DCF ) , troglitazone ( TGZ ) , and raloxifene , for which we observed known metabolic oxidation and bioconjugation pathways and turnover rates .
	manualset3
168735	6	412989	7	NULL	NULL	0	NULL	troglitazone ( TGZ )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The utility of the approach was illustrated by investigating the metabolism of the drugs diclofenac ( DCF ) , troglitazone ( TGZ ) , and raloxifene , for which we observed known metabolic oxidation and bioconjugation pathways and turnover rates .
	manualset3
168736	7	412989	7	NULL	NULL	0	NULL	raloxifene	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The utility of the approach was illustrated by investigating the metabolism of the drugs diclofenac ( DCF ) , troglitazone ( TGZ ) , and raloxifene , for which we observed known metabolic oxidation and bioconjugation pathways and turnover rates .
	manualset3
168737	8	412989	7	NULL	NULL	NULL	NULL	metabolic oxidation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The utility of the approach was illustrated by investigating the metabolism of the drugs diclofenac ( DCF ) , troglitazone ( TGZ ) , and raloxifene , for which we observed known metabolic oxidation and bioconjugation pathways and turnover rates .
	manualset3
168738	9	412989	7	NULL	NULL	NULL	NULL	bioconjugation pathways 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The utility of the approach was illustrated by investigating the metabolism of the drugs diclofenac ( DCF ) , troglitazone ( TGZ ) , and raloxifene , for which we observed known metabolic oxidation and bioconjugation pathways and turnover rates .
	manualset3
168739	10	412989	7	NULL	NULL	0	NULL	turnover rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The utility of the approach was illustrated by investigating the metabolism of the drugs diclofenac ( DCF ) , troglitazone ( TGZ ) , and raloxifene , for which we observed known metabolic oxidation and bioconjugation pathways and turnover rates .
	manualset3
168740	1	412990	7	NULL	NULL	0	NULL	utility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The utility of the dexamethasone suppression test ( DST ) in the diagnosis of depression was examined in an outpatient sample of 29 stroke patients .
	manualset3
168741	2	412990	7	NULL	NULL	0	NULL	dexamethasone suppression test ( DST )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The utility of the dexamethasone suppression test ( DST ) in the diagnosis of depression was examined in an outpatient sample of 29 stroke patients .
	manualset3
168742	3	412990	7	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The utility of the dexamethasone suppression test ( DST ) in the diagnosis of depression was examined in an outpatient sample of 29 stroke patients .
	manualset3
168743	4	412990	7	NULL	NULL	0	NULL	depression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The utility of the dexamethasone suppression test ( DST ) in the diagnosis of depression was examined in an outpatient sample of 29 stroke patients .
	manualset3
168744	5	412990	7	NULL	NULL	NULL	NULL	outpatient sample	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The utility of the dexamethasone suppression test ( DST ) in the diagnosis of depression was examined in an outpatient sample of 29 stroke patients .
	manualset3
168746	7	412990	7	NULL	NULL	0	NULL	29 stroke patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The utility of the dexamethasone suppression test ( DST ) in the diagnosis of depression was examined in an outpatient sample of 29 stroke patients .
	manualset3
168747	1	412991	7	NULL	NULL	0	NULL	utilization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The utilization of public networks could lead to the manipulation of data as well as undermine confidentiality .
	manualset3
168748	2	412991	7	NULL	NULL	0	NULL	public networks	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The utilization of public networks could lead to the manipulation of data as well as undermine confidentiality .
	manualset3
168749	3	412991	7	NULL	NULL	0	NULL	manipulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The utilization of public networks could lead to the manipulation of data as well as undermine confidentiality .
	manualset3
168750	4	412991	7	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The utilization of public networks could lead to the manipulation of data as well as undermine confidentiality .
	manualset3
168751	5	412991	7	NULL	NULL	0	NULL	confidentiality	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The utilization of public networks could lead to the manipulation of data as well as undermine confidentiality .
	manualset3
168752	1	412992	7	NULL	NULL	0	NULL	v-Myb protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The v-Myb protein binds to specific DNA sequences and can regulate gene expression .
	manualset3
168753	2	412992	7	NULL	NULL	0	NULL	DNA sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The v-Myb protein binds to specific DNA sequences and can regulate gene expression .
	manualset3
168754	3	412992	7	NULL	NULL	0	NULL	gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The v-Myb protein binds to specific DNA sequences and can regulate gene expression .
	manualset3
168755	1	412993	7	NULL	NULL	0	NULL	vaccine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The vaccine was well tolerated .
	manualset3
168756	1	412994	7	NULL	NULL	0	NULL	vacuolar membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The vacuolar membrane can form a large tubular invagination from which vesicles bud off into the lumen of the organelle .
	manualset3
168757	2	412994	7	NULL	NULL	NULL	NULL	large tubular invagination 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The vacuolar membrane can form a large tubular invagination from which vesicles bud off into the lumen of the organelle .
	manualset3
168758	3	412994	7	NULL	NULL	NULL	NULL	vesicles	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The vacuolar membrane can form a large tubular invagination from which vesicles bud off into the lumen of the organelle .
	manualset3
168759	4	412994	7	NULL	NULL	0	NULL	 lumen	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The vacuolar membrane can form a large tubular invagination from which vesicles bud off into the lumen of the organelle .
	manualset3
168760	5	412994	7	NULL	NULL	0	NULL	organelle	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The vacuolar membrane can form a large tubular invagination from which vesicles bud off into the lumen of the organelle .
	manualset3
168761	1	412995	7	NULL	NULL	NULL	NULL	Action	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Action of reserpine in morphine-tolerant rats : absence of an antagonism of catecholamine depletion .
	manualset3
168762	2	412995	7	NULL	NULL	0	NULL	reserpine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Action of reserpine in morphine-tolerant rats : absence of an antagonism of catecholamine depletion .
	manualset3
168763	3	412995	7	NULL	NULL	0	NULL	morphine-tolerant rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Action of reserpine in morphine-tolerant rats : absence of an antagonism of catecholamine depletion .
	manualset3
168764	4	412995	7	NULL	NULL	NULL	NULL	absence 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Action of reserpine in morphine-tolerant rats : absence of an antagonism of catecholamine depletion .
	manualset3
168765	5	412995	7	NULL	NULL	NULL	NULL	antagonism	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Action of reserpine in morphine-tolerant rats : absence of an antagonism of catecholamine depletion .
	manualset3
168766	6	412995	7	NULL	NULL	NULL	NULL	catecholamine depletion	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Action of reserpine in morphine-tolerant rats : absence of an antagonism of catecholamine depletion .
	manualset3
168767	1	412996	7	NULL	NULL	NULL	NULL	valence shell photoelectron spectrum	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The valence shell photoelectron spectrum , threshold photoelectron spectrum , and threshold photoelectron photoion coincidence ( TPEPICO ) mass spectra of acetone have been measured using synchrotron radiation .
	manualset3
168768	2	412996	7	NULL	NULL	NULL	NULL	threshold photoelectron spectrum	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The valence shell photoelectron spectrum , threshold photoelectron spectrum , and threshold photoelectron photoion coincidence ( TPEPICO ) mass spectra of acetone have been measured using synchrotron radiation .
	manualset3
168769	3	412996	7	NULL	NULL	NULL	NULL	threshold photoelectron photoion coincidence ( TPEPICO ) mass spectra of acetone	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The valence shell photoelectron spectrum , threshold photoelectron spectrum , and threshold photoelectron photoion coincidence ( TPEPICO ) mass spectra of acetone have been measured using synchrotron radiation .
	manualset3
168771	4	412996	7	NULL	NULL	NULL	NULL	synchrotron radiation	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The valence shell photoelectron spectrum , threshold photoelectron spectrum , and threshold photoelectron photoion coincidence ( TPEPICO ) mass spectra of acetone have been measured using synchrotron radiation .
	manualset3
168772	1	412997	7	NULL	NULL	0	NULL	validation outcome	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The validation outcome showed that each assay was robust , reliable and accurate to meet the requirements of the intended analytical application , that being to 1 ) quantitatively determine the concentration of antibody in the serum and 2 ) determine whether a sample is positive or negative for human anti-chimeric antibodies .
	manualset3
168773	2	412997	7	NULL	NULL	0	NULL	assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The validation outcome showed that each assay was robust , reliable and accurate to meet the requirements of the intended analytical application , that being to 1 ) quantitatively determine the concentration of antibody in the serum and 2 ) determine whether a sample is positive or negative for human anti-chimeric antibodies .
	manualset3
168774	3	412997	7	NULL	NULL	0	NULL	requirements	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The validation outcome showed that each assay was robust , reliable and accurate to meet the requirements of the intended analytical application , that being to 1 ) quantitatively determine the concentration of antibody in the serum and 2 ) determine whether a sample is positive or negative for human anti-chimeric antibodies .
	manualset3
168775	4	412997	7	NULL	NULL	0	NULL	intended analytical application	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The validation outcome showed that each assay was robust , reliable and accurate to meet the requirements of the intended analytical application , that being to 1 ) quantitatively determine the concentration of antibody in the serum and 2 ) determine whether a sample is positive or negative for human anti-chimeric antibodies .
	manualset3
168776	5	412997	7	NULL	NULL	0	NULL	 concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The validation outcome showed that each assay was robust , reliable and accurate to meet the requirements of the intended analytical application , that being to 1 ) quantitatively determine the concentration of antibody in the serum and 2 ) determine whether a sample is positive or negative for human anti-chimeric antibodies .
	manualset3
168777	6	412997	7	NULL	NULL	0	NULL	antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The validation outcome showed that each assay was robust , reliable and accurate to meet the requirements of the intended analytical application , that being to 1 ) quantitatively determine the concentration of antibody in the serum and 2 ) determine whether a sample is positive or negative for human anti-chimeric antibodies .
	manualset3
168778	7	412997	7	NULL	NULL	0	NULL	serum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The validation outcome showed that each assay was robust , reliable and accurate to meet the requirements of the intended analytical application , that being to 1 ) quantitatively determine the concentration of antibody in the serum and 2 ) determine whether a sample is positive or negative for human anti-chimeric antibodies .
	manualset3
168779	8	412997	7	NULL	NULL	0	NULL	sample	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The validation outcome showed that each assay was robust , reliable and accurate to meet the requirements of the intended analytical application , that being to 1 ) quantitatively determine the concentration of antibody in the serum and 2 ) determine whether a sample is positive or negative for human anti-chimeric antibodies .
	manualset3
168780	9	412997	7	NULL	NULL	0	NULL	human anti-chimeric antibodies	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The validation outcome showed that each assay was robust , reliable and accurate to meet the requirements of the intended analytical application , that being to 1 ) quantitatively determine the concentration of antibody in the serum and 2 ) determine whether a sample is positive or negative for human anti-chimeric antibodies .
	manualset3
168781	1	412998	7	NULL	NULL	0	NULL	validity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The validity of this typing procedure was confirmed by the identification of all DRB alleles previously characterized by cloning and sequencing techniques from an individual cotton-top tamarin .
	manualset3
168783	2	412998	7	NULL	NULL	0	NULL	typing procedure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The validity of this typing procedure was confirmed by the identification of all DRB alleles previously characterized by cloning and sequencing techniques from an individual cotton-top tamarin .
	manualset3
168784	3	412998	7	NULL	NULL	0	NULL	 identification 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The validity of this typing procedure was confirmed by the identification of all DRB alleles previously characterized by cloning and sequencing techniques from an individual cotton-top tamarin .
	manualset3
168785	4	412998	7	NULL	NULL	0	NULL	DRB alleles	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The validity of this typing procedure was confirmed by the identification of all DRB alleles previously characterized by cloning and sequencing techniques from an individual cotton-top tamarin .
	manualset3
168786	5	412998	7	NULL	NULL	0	NULL	cloning technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The validity of this typing procedure was confirmed by the identification of all DRB alleles previously characterized by cloning and sequencing techniques from an individual cotton-top tamarin .
	manualset3
168787	6	412998	7	NULL	NULL	0	NULL	sequencing technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The validity of this typing procedure was confirmed by the identification of all DRB alleles previously characterized by cloning and sequencing techniques from an individual cotton-top tamarin .
	manualset3
168788	7	412998	7	NULL	NULL	0	NULL	individual 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The validity of this typing procedure was confirmed by the identification of all DRB alleles previously characterized by cloning and sequencing techniques from an individual cotton-top tamarin .
	manualset3
168789	8	412998	7	NULL	NULL	0	NULL	cotton-top tamarin .	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The validity of this typing procedure was confirmed by the identification of all DRB alleles previously characterized by cloning and sequencing techniques from an individual cotton-top tamarin .
	manualset3
168790	1	412999	7	NULL	NULL	0	NULL	validity	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The validity of twelve provocative tests for carpal tunnel syndrome ( CTS ) in a random sample of 504 people from the general population was assessed .
	manualset3
168791	2	412999	7	NULL	NULL	0	NULL	twelve provocative tests	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The validity of twelve provocative tests for carpal tunnel syndrome ( CTS ) in a random sample of 504 people from the general population was assessed .
	manualset3
168792	3	412999	7	NULL	NULL	0	NULL	carpal tunnel syndrome ( CTS )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The validity of twelve provocative tests for carpal tunnel syndrome ( CTS ) in a random sample of 504 people from the general population was assessed .
	manualset3
168793	4	412999	7	NULL	NULL	0	NULL	random sample	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The validity of twelve provocative tests for carpal tunnel syndrome ( CTS ) in a random sample of 504 people from the general population was assessed .
	manualset3
168794	5	412999	7	NULL	NULL	0	NULL	504 people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The validity of twelve provocative tests for carpal tunnel syndrome ( CTS ) in a random sample of 504 people from the general population was assessed .
	manualset3
168795	6	412999	7	NULL	NULL	0	NULL	general population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The validity of twelve provocative tests for carpal tunnel syndrome ( CTS ) in a random sample of 504 people from the general population was assessed .
	manualset3
168796	1	413000	7	NULL	NULL	0	NULL	value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The value of a `` bread-barium '' swallow for diagnosis of disordered esophageal motility was examined in 53 patients , 20 of whom complained of dysphagia , 20 retrosternal chest pain , and 13 heartburn ; a further 19 subjects served as controls .
	manualset3
168797	2	413000	7	NULL	NULL	NULL	NULL	 bread-barium '' swallow	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The value of a `` bread-barium '' swallow for diagnosis of disordered esophageal motility was examined in 53 patients , 20 of whom complained of dysphagia , 20 retrosternal chest pain , and 13 heartburn ; a further 19 subjects served as controls .
	manualset3
168798	3	413000	7	NULL	NULL	0	NULL	diagnosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The value of a `` bread-barium '' swallow for diagnosis of disordered esophageal motility was examined in 53 patients , 20 of whom complained of dysphagia , 20 retrosternal chest pain , and 13 heartburn ; a further 19 subjects served as controls .
	manualset3
168799	4	413000	7	NULL	NULL	0	NULL	disordered esophageal motility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The value of a `` bread-barium '' swallow for diagnosis of disordered esophageal motility was examined in 53 patients , 20 of whom complained of dysphagia , 20 retrosternal chest pain , and 13 heartburn ; a further 19 subjects served as controls .
	manualset3
168800	5	413000	7	NULL	NULL	0	NULL	53 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The value of a `` bread-barium '' swallow for diagnosis of disordered esophageal motility was examined in 53 patients , 20 of whom complained of dysphagia , 20 retrosternal chest pain , and 13 heartburn ; a further 19 subjects served as controls .
	manualset3
168801	6	413000	7	NULL	NULL	NULL	NULL	 20	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The value of a `` bread-barium '' swallow for diagnosis of disordered esophageal motility was examined in 53 patients , 20 of whom complained of dysphagia , 20 retrosternal chest pain , and 13 heartburn ; a further 19 subjects served as controls .
	manualset3
168802	7	413000	7	NULL	NULL	0	NULL	dysphagia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The value of a `` bread-barium '' swallow for diagnosis of disordered esophageal motility was examined in 53 patients , 20 of whom complained of dysphagia , 20 retrosternal chest pain , and 13 heartburn ; a further 19 subjects served as controls .
	manualset3
168803	8	413000	7	NULL	NULL	0	NULL	 20	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The value of a `` bread-barium '' swallow for diagnosis of disordered esophageal motility was examined in 53 patients , 20 of whom complained of dysphagia , 20 retrosternal chest pain , and 13 heartburn ; a further 19 subjects served as controls .
	manualset3
168804	9	413000	7	NULL	NULL	0	NULL	retrosternal chest pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The value of a `` bread-barium '' swallow for diagnosis of disordered esophageal motility was examined in 53 patients , 20 of whom complained of dysphagia , 20 retrosternal chest pain , and 13 heartburn ; a further 19 subjects served as controls .
	manualset3
168805	10	413000	7	NULL	NULL	0	NULL	13	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The value of a `` bread-barium '' swallow for diagnosis of disordered esophageal motility was examined in 53 patients , 20 of whom complained of dysphagia , 20 retrosternal chest pain , and 13 heartburn ; a further 19 subjects served as controls .
	manualset3
168806	11	413000	7	NULL	NULL	0	NULL	heartburn	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The value of a `` bread-barium '' swallow for diagnosis of disordered esophageal motility was examined in 53 patients , 20 of whom complained of dysphagia , 20 retrosternal chest pain , and 13 heartburn ; a further 19 subjects served as controls .
	manualset3
168807	12	413000	7	NULL	NULL	0	NULL	19 subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The value of a `` bread-barium '' swallow for diagnosis of disordered esophageal motility was examined in 53 patients , 20 of whom complained of dysphagia , 20 retrosternal chest pain , and 13 heartburn ; a further 19 subjects served as controls .
	manualset3
168808	13	413000	7	NULL	NULL	0	NULL	controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The value of a `` bread-barium '' swallow for diagnosis of disordered esophageal motility was examined in 53 patients , 20 of whom complained of dysphagia , 20 retrosternal chest pain , and 13 heartburn ; a further 19 subjects served as controls .
	manualset3
168809	1	413001	7	NULL	NULL	0	NULL	value	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The value of postmortem computed tomography as an alternative for autopsy in trauma victims : a systematic review .
	manualset3
168810	2	413001	7	NULL	NULL	NULL	NULL	postmortem computed tomography	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The value of postmortem computed tomography as an alternative for autopsy in trauma victims : a systematic review .
	manualset3
168811	3	413001	7	NULL	NULL	0	NULL	autopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The value of postmortem computed tomography as an alternative for autopsy in trauma victims : a systematic review .
	manualset3
168812	4	413001	7	NULL	NULL	0	NULL	trauma victims	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The value of postmortem computed tomography as an alternative for autopsy in trauma victims : a systematic review .
	manualset3
168813	5	413001	7	NULL	NULL	0	NULL	systematic review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The value of postmortem computed tomography as an alternative for autopsy in trauma victims : a systematic review .
	manualset3
170376	6	413001	7	NULL	NULL	0	NULL	alternative	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The value of postmortem computed tomography as an alternative for autopsy in trauma victims : a systematic review .
	manualset3
168814	1	413002	7	NULL	NULL	0	NULL	value	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The value of somatostatin-receptor scintigraphy in newly diagnosed endocrine gastroenteropancreatic tumors .
	manualset3
168815	2	413002	7	NULL	NULL	NULL	NULL	somatostatin-receptor scintigraphy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The value of somatostatin-receptor scintigraphy in newly diagnosed endocrine gastroenteropancreatic tumors .
	manualset3
168816	3	413002	7	NULL	NULL	0	NULL	endocrine gastroenteropancreatic tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The value of somatostatin-receptor scintigraphy in newly diagnosed endocrine gastroenteropancreatic tumors .
	manualset3
168817	1	413003	7	NULL	NULL	0	NULL	Combination chemical therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Combination chemical and roentgenographic therapy in certain malignant tumors ) .
	manualset3
168818	2	413003	7	NULL	NULL	0	NULL	roentgenographic therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Combination chemical and roentgenographic therapy in certain malignant tumors ) .
	manualset3
168819	3	413003	7	NULL	NULL	0	NULL	malignant tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Combination chemical and roentgenographic therapy in certain malignant tumors ) .
	manualset3
168820	1	413004	7	NULL	NULL	0	NULL	Activated T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Activated T cells up-regulate CLA expression , but little is currently known about their binding to P-selectin .
	manualset3
168821	2	413004	7	NULL	NULL	0	NULL	CLA expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activated T cells up-regulate CLA expression , but little is currently known about their binding to P-selectin .
	manualset3
168822	3	413004	7	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activated T cells up-regulate CLA expression , but little is currently known about their binding to P-selectin .
	manualset3
168823	4	413004	7	NULL	NULL	0	NULL	P-selectin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Activated T cells up-regulate CLA expression , but little is currently known about their binding to P-selectin .
	manualset3
168824	1	413005	7	NULL	NULL	0	NULL	values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The values from our assay correlated well with total renin activity measured as the generation rate of angiotensin I after trypsin activation ( r = 0.78 , p less than 0.01 ) , but correlated weakly with active renin activity .
	manualset3
168825	2	413005	7	NULL	NULL	0	NULL	assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The values from our assay correlated well with total renin activity measured as the generation rate of angiotensin I after trypsin activation ( r = 0.78 , p less than 0.01 ) , but correlated weakly with active renin activity .
	manualset3
168826	3	413005	7	NULL	NULL	0	NULL	total renin activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The values from our assay correlated well with total renin activity measured as the generation rate of angiotensin I after trypsin activation ( r = 0.78 , p less than 0.01 ) , but correlated weakly with active renin activity .
	manualset3
168827	4	413005	7	NULL	NULL	0	NULL	generation rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The values from our assay correlated well with total renin activity measured as the generation rate of angiotensin I after trypsin activation ( r = 0.78 , p less than 0.01 ) , but correlated weakly with active renin activity .
	manualset3
168828	5	413005	7	NULL	NULL	0	NULL	angiotensin I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The values from our assay correlated well with total renin activity measured as the generation rate of angiotensin I after trypsin activation ( r = 0.78 , p less than 0.01 ) , but correlated weakly with active renin activity .
	manualset3
168829	6	413005	7	NULL	NULL	0	NULL	trypsin activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The values from our assay correlated well with total renin activity measured as the generation rate of angiotensin I after trypsin activation ( r = 0.78 , p less than 0.01 ) , but correlated weakly with active renin activity .
	manualset3
168830	7	413005	7	NULL	NULL	0	NULL	r = 0.78 , p less than 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The values from our assay correlated well with total renin activity measured as the generation rate of angiotensin I after trypsin activation ( r = 0.78 , p less than 0.01 ) , but correlated weakly with active renin activity .
	manualset3
168831	8	413005	7	NULL	NULL	0	NULL	active renin activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The values from our assay correlated well with total renin activity measured as the generation rate of angiotensin I after trypsin activation ( r = 0.78 , p less than 0.01 ) , but correlated weakly with active renin activity .
	manualset3
168832	1	413006	7	NULL	NULL	0	NULL	values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The values of immunoglobulin classes IgA and IgG , coplement , enzymatic activity of total acid phosphatase and sorbitodechydrogenase and `` acute phase '' proteins were established to be with regularly increased values with high statistical significance .
	manualset3
168833	2	413006	7	NULL	NULL	0	NULL	immunoglobulin classes IgA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The values of immunoglobulin classes IgA and IgG , coplement , enzymatic activity of total acid phosphatase and sorbitodechydrogenase and `` acute phase '' proteins were established to be with regularly increased values with high statistical significance .
	manualset3
168834	3	413006	7	NULL	NULL	0	NULL	immunoglobulin classes IgG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The values of immunoglobulin classes IgA and IgG , coplement , enzymatic activity of total acid phosphatase and sorbitodechydrogenase and `` acute phase '' proteins were established to be with regularly increased values with high statistical significance .
	manualset3
168835	4	413006	7	NULL	NULL	0	NULL	coplement 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The values of immunoglobulin classes IgA and IgG , coplement , enzymatic activity of total acid phosphatase and sorbitodechydrogenase and `` acute phase '' proteins were established to be with regularly increased values with high statistical significance .
	manualset3
168836	5	413006	7	NULL	NULL	0	NULL	enzymatic activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The values of immunoglobulin classes IgA and IgG , coplement , enzymatic activity of total acid phosphatase and sorbitodechydrogenase and `` acute phase '' proteins were established to be with regularly increased values with high statistical significance .
	manualset3
168837	6	413006	7	NULL	NULL	0	NULL	 total acid phosphatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The values of immunoglobulin classes IgA and IgG , coplement , enzymatic activity of total acid phosphatase and sorbitodechydrogenase and `` acute phase '' proteins were established to be with regularly increased values with high statistical significance .
	manualset3
168838	7	413006	7	NULL	NULL	0	NULL	sorbitodechydrogenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The values of immunoglobulin classes IgA and IgG , coplement , enzymatic activity of total acid phosphatase and sorbitodechydrogenase and `` acute phase '' proteins were established to be with regularly increased values with high statistical significance .
	manualset3
168839	8	413006	7	NULL	NULL	0	NULL	`` acute phase '' proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The values of immunoglobulin classes IgA and IgG , coplement , enzymatic activity of total acid phosphatase and sorbitodechydrogenase and `` acute phase '' proteins were established to be with regularly increased values with high statistical significance .
	manualset3
168840	9	413006	7	NULL	NULL	0	NULL	increased values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The values of immunoglobulin classes IgA and IgG , coplement , enzymatic activity of total acid phosphatase and sorbitodechydrogenase and `` acute phase '' proteins were established to be with regularly increased values with high statistical significance .
	manualset3
168841	10	413006	7	NULL	NULL	0	NULL	high statistical significance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The values of immunoglobulin classes IgA and IgG , coplement , enzymatic activity of total acid phosphatase and sorbitodechydrogenase and `` acute phase '' proteins were established to be with regularly increased values with high statistical significance .
	manualset3
168842	1	413007	7	NULL	NULL	0	NULL	values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The values of the critical exponents suggest that long-range interactions are present in the SmCalpha * - SmC * critical region .
	manualset3
168843	2	413007	7	NULL	NULL	0	NULL	critical exponents	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The values of the critical exponents suggest that long-range interactions are present in the SmCalpha * - SmC * critical region .
	manualset3
168844	3	413007	7	NULL	NULL	0	NULL	 long-range interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The values of the critical exponents suggest that long-range interactions are present in the SmCalpha * - SmC * critical region .
	manualset3
168845	4	413007	7	NULL	NULL	0	NULL	SmCalpha * - SmC * critical region 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The values of the critical exponents suggest that long-range interactions are present in the SmCalpha * - SmC * critical region .
	manualset3
168846	1	413008	7	NULL	NULL	0	NULL	 variability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The variability of the HLA antigens is given by the presence of many alleles of the HLA genes .
	manualset3
168847	2	413008	7	NULL	NULL	0	NULL	HLA antigens	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The variability of the HLA antigens is given by the presence of many alleles of the HLA genes .
	manualset3
168848	3	413008	7	NULL	NULL	0	NULL	alleles	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The variability of the HLA antigens is given by the presence of many alleles of the HLA genes .
	manualset3
168849	4	413008	7	NULL	NULL	0	NULL	HLA genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The variability of the HLA antigens is given by the presence of many alleles of the HLA genes .
	manualset3
168850	1	413009	7	NULL	NULL	0	NULL	Activated c-Cbl	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Activated c-Cbl localized with LRs at the junctional base of macropinocytic blebs .
	manualset3
168851	2	413009	7	NULL	NULL	0	NULL	LRs 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Activated c-Cbl localized with LRs at the junctional base of macropinocytic blebs .
	manualset3
168852	3	413009	7	NULL	NULL	0	NULL	 junctional base	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Activated c-Cbl localized with LRs at the junctional base of macropinocytic blebs .
	manualset3
168853	4	413009	7	NULL	NULL	0	NULL	macropinocytic blebs	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Activated c-Cbl localized with LRs at the junctional base of macropinocytic blebs .
	manualset3
168854	1	413010	7	NULL	NULL	0	NULL	 variables	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The variables influencing the extraction ( amplitude of the ultrasound pulse , the extraction time and the solvent ) were studied by a full factorial design and a central composite design .
	manualset3
168855	2	413010	7	NULL	NULL	0	NULL	extraction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The variables influencing the extraction ( amplitude of the ultrasound pulse , the extraction time and the solvent ) were studied by a full factorial design and a central composite design .
	manualset3
168856	3	413010	7	NULL	NULL	0	NULL	amplitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The variables influencing the extraction ( amplitude of the ultrasound pulse , the extraction time and the solvent ) were studied by a full factorial design and a central composite design .
	manualset3
168857	4	413010	7	NULL	NULL	0	NULL	ultrasound pulse	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The variables influencing the extraction ( amplitude of the ultrasound pulse , the extraction time and the solvent ) were studied by a full factorial design and a central composite design .
	manualset3
168858	5	413010	7	NULL	NULL	0	NULL	extraction time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The variables influencing the extraction ( amplitude of the ultrasound pulse , the extraction time and the solvent ) were studied by a full factorial design and a central composite design .
	manualset3
168859	7	413010	7	NULL	NULL	NULL	NULL	full factorial design	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The variables influencing the extraction ( amplitude of the ultrasound pulse , the extraction time and the solvent ) were studied by a full factorial design and a central composite design .
	manualset3
168860	8	413010	7	NULL	NULL	NULL	NULL	central composite design 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The variables influencing the extraction ( amplitude of the ultrasound pulse , the extraction time and the solvent ) were studied by a full factorial design and a central composite design .
	manualset3
168861	6	413010	7	NULL	NULL	0	NULL	solvent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The variables influencing the extraction ( amplitude of the ultrasound pulse , the extraction time and the solvent ) were studied by a full factorial design and a central composite design .
	manualset3
168862	1	413011	7	NULL	NULL	0	NULL	 variables	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The variables without significant effect on sex ratio were : age , sex , clinical status and sickle cell trait status of the gametocyte carrier , density of asexual parasites , quinine treatment , and gametocyte density ( when taking account of its waves ) .
	manualset3
168863	2	413011	7	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The variables without significant effect on sex ratio were : age , sex , clinical status and sickle cell trait status of the gametocyte carrier , density of asexual parasites , quinine treatment , and gametocyte density ( when taking account of its waves ) .
	manualset3
168864	3	413011	7	NULL	NULL	0	NULL	sex ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The variables without significant effect on sex ratio were : age , sex , clinical status and sickle cell trait status of the gametocyte carrier , density of asexual parasites , quinine treatment , and gametocyte density ( when taking account of its waves ) .
	manualset3
168865	4	413011	7	NULL	NULL	0	NULL	age	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The variables without significant effect on sex ratio were : age , sex , clinical status and sickle cell trait status of the gametocyte carrier , density of asexual parasites , quinine treatment , and gametocyte density ( when taking account of its waves ) .
	manualset3
168866	5	413011	7	NULL	NULL	0	NULL	sex	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The variables without significant effect on sex ratio were : age , sex , clinical status and sickle cell trait status of the gametocyte carrier , density of asexual parasites , quinine treatment , and gametocyte density ( when taking account of its waves ) .
	manualset3
168867	6	413011	7	NULL	NULL	0	NULL	 clinical status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The variables without significant effect on sex ratio were : age , sex , clinical status and sickle cell trait status of the gametocyte carrier , density of asexual parasites , quinine treatment , and gametocyte density ( when taking account of its waves ) .
	manualset3
168868	7	413011	7	NULL	NULL	0	NULL	sickle cell trait status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The variables without significant effect on sex ratio were : age , sex , clinical status and sickle cell trait status of the gametocyte carrier , density of asexual parasites , quinine treatment , and gametocyte density ( when taking account of its waves ) .
	manualset3
168869	8	413011	7	NULL	NULL	0	NULL	 gametocyte carrier	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The variables without significant effect on sex ratio were : age , sex , clinical status and sickle cell trait status of the gametocyte carrier , density of asexual parasites , quinine treatment , and gametocyte density ( when taking account of its waves ) .
	manualset3
168870	9	413011	7	NULL	NULL	0	NULL	 density	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The variables without significant effect on sex ratio were : age , sex , clinical status and sickle cell trait status of the gametocyte carrier , density of asexual parasites , quinine treatment , and gametocyte density ( when taking account of its waves ) .
	manualset3
168871	10	413011	7	NULL	NULL	0	NULL	asexual parasites	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The variables without significant effect on sex ratio were : age , sex , clinical status and sickle cell trait status of the gametocyte carrier , density of asexual parasites , quinine treatment , and gametocyte density ( when taking account of its waves ) .
	manualset3
168872	11	413011	7	NULL	NULL	0	NULL	quinine treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The variables without significant effect on sex ratio were : age , sex , clinical status and sickle cell trait status of the gametocyte carrier , density of asexual parasites , quinine treatment , and gametocyte density ( when taking account of its waves ) .
	manualset3
168873	12	413011	7	NULL	NULL	0	NULL	gametocyte density	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The variables without significant effect on sex ratio were : age , sex , clinical status and sickle cell trait status of the gametocyte carrier , density of asexual parasites , quinine treatment , and gametocyte density ( when taking account of its waves ) .
	manualset3
168874	13	413011	7	NULL	NULL	0	NULL	waves	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The variables without significant effect on sex ratio were : age , sex , clinical status and sickle cell trait status of the gametocyte carrier , density of asexual parasites , quinine treatment , and gametocyte density ( when taking account of its waves ) .
	manualset3
168895	1	413012	7	NULL	NULL	0	NULL	variance	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The variance was less than in adults .5 .
	manualset3
168896	2	413012	7	NULL	NULL	0	NULL	adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The variance was less than in adults .5 .
	manualset3
168897	3	413012	7	NULL	NULL	0	NULL	 .5 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The variance was less than in adults .5 .
	manualset3
169046	1	413013	7	NULL	NULL	0	NULL	 variation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The variation of heading thresholds from radial to lamellar flow fields is predicted by a simple model of two-dimensional motion discrimination .
	manualset3
169047	2	413013	7	NULL	NULL	0	NULL	heading thresholds	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The variation of heading thresholds from radial to lamellar flow fields is predicted by a simple model of two-dimensional motion discrimination .
	manualset3
169048	3	413013	7	NULL	NULL	0	NULL	radial field	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The variation of heading thresholds from radial to lamellar flow fields is predicted by a simple model of two-dimensional motion discrimination .
	manualset3
169049	4	413013	7	NULL	NULL	0	NULL	lamellar flow fields 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The variation of heading thresholds from radial to lamellar flow fields is predicted by a simple model of two-dimensional motion discrimination .
	manualset3
169050	5	413013	7	NULL	NULL	0	NULL	simple model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The variation of heading thresholds from radial to lamellar flow fields is predicted by a simple model of two-dimensional motion discrimination .
	manualset3
169051	6	413013	7	NULL	NULL	0	NULL	two-dimensional motion discrimination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The variation of heading thresholds from radial to lamellar flow fields is predicted by a simple model of two-dimensional motion discrimination .
	manualset3
169052	1	413014	7	NULL	NULL	0	NULL	 variations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The variations in plasma levels of TSH , T4 , T3 , and rT3 , during the pubertal period , were studied in 647 school students from the urban area of Santiago in Chile ( 47 % males and 53 % females ) with ages ranging between 7.5 and 15 yr .
	manualset3
169053	2	413014	7	NULL	NULL	0	NULL	plasma levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The variations in plasma levels of TSH , T4 , T3 , and rT3 , during the pubertal period , were studied in 647 school students from the urban area of Santiago in Chile ( 47 % males and 53 % females ) with ages ranging between 7.5 and 15 yr .
	manualset3
169054	3	413014	7	NULL	NULL	0	NULL	 TSH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The variations in plasma levels of TSH , T4 , T3 , and rT3 , during the pubertal period , were studied in 647 school students from the urban area of Santiago in Chile ( 47 % males and 53 % females ) with ages ranging between 7.5 and 15 yr .
	manualset3
169055	4	413014	7	NULL	NULL	0	NULL	T4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The variations in plasma levels of TSH , T4 , T3 , and rT3 , during the pubertal period , were studied in 647 school students from the urban area of Santiago in Chile ( 47 % males and 53 % females ) with ages ranging between 7.5 and 15 yr .
	manualset3
169056	5	413014	7	NULL	NULL	0	NULL	T3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The variations in plasma levels of TSH , T4 , T3 , and rT3 , during the pubertal period , were studied in 647 school students from the urban area of Santiago in Chile ( 47 % males and 53 % females ) with ages ranging between 7.5 and 15 yr .
	manualset3
169057	6	413014	7	NULL	NULL	0	NULL	rT3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The variations in plasma levels of TSH , T4 , T3 , and rT3 , during the pubertal period , were studied in 647 school students from the urban area of Santiago in Chile ( 47 % males and 53 % females ) with ages ranging between 7.5 and 15 yr .
	manualset3
169058	7	413014	7	NULL	NULL	0	NULL	pubertal period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The variations in plasma levels of TSH , T4 , T3 , and rT3 , during the pubertal period , were studied in 647 school students from the urban area of Santiago in Chile ( 47 % males and 53 % females ) with ages ranging between 7.5 and 15 yr .
	manualset3
169059	8	413014	7	NULL	NULL	0	NULL	647	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The variations in plasma levels of TSH , T4 , T3 , and rT3 , during the pubertal period , were studied in 647 school students from the urban area of Santiago in Chile ( 47 % males and 53 % females ) with ages ranging between 7.5 and 15 yr .
	manualset3
169060	9	413014	7	NULL	NULL	0	NULL	school students	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The variations in plasma levels of TSH , T4 , T3 , and rT3 , during the pubertal period , were studied in 647 school students from the urban area of Santiago in Chile ( 47 % males and 53 % females ) with ages ranging between 7.5 and 15 yr .
	manualset3
169061	10	413014	7	NULL	NULL	NULL	NULL	urban area 	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The variations in plasma levels of TSH , T4 , T3 , and rT3 , during the pubertal period , were studied in 647 school students from the urban area of Santiago in Chile ( 47 % males and 53 % females ) with ages ranging between 7.5 and 15 yr .
	manualset3
169062	11	413014	7	NULL	NULL	0	NULL	Santiago	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The variations in plasma levels of TSH , T4 , T3 , and rT3 , during the pubertal period , were studied in 647 school students from the urban area of Santiago in Chile ( 47 % males and 53 % females ) with ages ranging between 7.5 and 15 yr .
	manualset3
169063	12	413014	7	NULL	NULL	0	NULL	Chile	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The variations in plasma levels of TSH , T4 , T3 , and rT3 , during the pubertal period , were studied in 647 school students from the urban area of Santiago in Chile ( 47 % males and 53 % females ) with ages ranging between 7.5 and 15 yr .
	manualset3
169064	13	413014	7	NULL	NULL	0	NULL	 47 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The variations in plasma levels of TSH , T4 , T3 , and rT3 , during the pubertal period , were studied in 647 school students from the urban area of Santiago in Chile ( 47 % males and 53 % females ) with ages ranging between 7.5 and 15 yr .
	manualset3
169065	14	413014	7	NULL	NULL	0	NULL	males	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The variations in plasma levels of TSH , T4 , T3 , and rT3 , during the pubertal period , were studied in 647 school students from the urban area of Santiago in Chile ( 47 % males and 53 % females ) with ages ranging between 7.5 and 15 yr .
	manualset3
169066	15	413014	7	NULL	NULL	0	NULL	 53 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The variations in plasma levels of TSH , T4 , T3 , and rT3 , during the pubertal period , were studied in 647 school students from the urban area of Santiago in Chile ( 47 % males and 53 % females ) with ages ranging between 7.5 and 15 yr .
	manualset3
169067	16	413014	7	NULL	NULL	0	NULL	females	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The variations in plasma levels of TSH , T4 , T3 , and rT3 , during the pubertal period , were studied in 647 school students from the urban area of Santiago in Chile ( 47 % males and 53 % females ) with ages ranging between 7.5 and 15 yr .
	manualset3
169068	17	413014	7	NULL	NULL	0	NULL	ages	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The variations in plasma levels of TSH , T4 , T3 , and rT3 , during the pubertal period , were studied in 647 school students from the urban area of Santiago in Chile ( 47 % males and 53 % females ) with ages ranging between 7.5 and 15 yr .
	manualset3
169069	18	413014	7	NULL	NULL	0	NULL	7.5 yr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The variations in plasma levels of TSH , T4 , T3 , and rT3 , during the pubertal period , were studied in 647 school students from the urban area of Santiago in Chile ( 47 % males and 53 % females ) with ages ranging between 7.5 and 15 yr .
	manualset3
169070	19	413014	7	NULL	NULL	0	NULL	15 yr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The variations in plasma levels of TSH , T4 , T3 , and rT3 , during the pubertal period , were studied in 647 school students from the urban area of Santiago in Chile ( 47 % males and 53 % females ) with ages ranging between 7.5 and 15 yr .
	manualset3
169071	1	413015	7	NULL	NULL	0	NULL	 varieties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The varieties of brain abscess seen in Papua New Guinea are very much those seen by Sir William Macewen a century ago .
	manualset3
169072	2	413015	7	NULL	NULL	0	NULL	brain abscess	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The varieties of brain abscess seen in Papua New Guinea are very much those seen by Sir William Macewen a century ago .
	manualset3
169073	3	413015	7	NULL	NULL	0	NULL	Papua New Guinea	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The varieties of brain abscess seen in Papua New Guinea are very much those seen by Sir William Macewen a century ago .
	manualset3
169074	4	413015	7	NULL	NULL	0	NULL	Sir William Macewen	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The varieties of brain abscess seen in Papua New Guinea are very much those seen by Sir William Macewen a century ago .
	manualset3
169075	5	413015	7	NULL	NULL	0	NULL	century ago	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The varieties of brain abscess seen in Papua New Guinea are very much those seen by Sir William Macewen a century ago .
	manualset3
169076	1	413016	7	NULL	NULL	NULL	NULL	cytokine responses	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The various cytokine responses associated with stimulation by parasites is discussed with emphasis on Leishmania parasites .
	manualset3
169077	2	413016	7	NULL	NULL	NULL	NULL	stimulation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The various cytokine responses associated with stimulation by parasites is discussed with emphasis on Leishmania parasites .
	manualset3
169078	3	413016	7	NULL	NULL	0	NULL	 parasites	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The various cytokine responses associated with stimulation by parasites is discussed with emphasis on Leishmania parasites .
	manualset3
169079	5	413016	7	NULL	NULL	NULL	NULL	Leishmania parasites	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The various cytokine responses associated with stimulation by parasites is discussed with emphasis on Leishmania parasites .
	manualset3
169080	4	413016	7	NULL	NULL	0	NULL	emphasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The various cytokine responses associated with stimulation by parasites is discussed with emphasis on Leishmania parasites .
	manualset3
169081	1	413017	7	NULL	NULL	0	NULL	Activated spermatozoa	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Activated spermatozoa are only found in the uterus internus of females , which is an indication of internal fertilization .
	manualset3
169082	2	413017	7	NULL	NULL	0	NULL	uterus internus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Activated spermatozoa are only found in the uterus internus of females , which is an indication of internal fertilization .
	manualset3
169083	3	413017	7	NULL	NULL	0	NULL	females	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Activated spermatozoa are only found in the uterus internus of females , which is an indication of internal fertilization .
	manualset3
169084	4	413017	7	NULL	NULL	0	NULL	indication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Activated spermatozoa are only found in the uterus internus of females , which is an indication of internal fertilization .
	manualset3
169085	5	413017	7	NULL	NULL	0	NULL	internal fertilization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activated spermatozoa are only found in the uterus internus of females , which is an indication of internal fertilization .
	manualset3
169086	1	413018	7	NULL	NULL	0	NULL	 various factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The various factors that can cause a mouthbreathing habit , such as asthma , allergies and enlarged glandular tissue , are discussed in detail .
	manualset3
169087	2	413018	7	NULL	NULL	0	NULL	mouthbreathing habit	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The various factors that can cause a mouthbreathing habit , such as asthma , allergies and enlarged glandular tissue , are discussed in detail .
	manualset3
169088	3	413018	7	NULL	NULL	0	NULL	asthma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The various factors that can cause a mouthbreathing habit , such as asthma , allergies and enlarged glandular tissue , are discussed in detail .
	manualset3
169089	4	413018	7	NULL	NULL	0	NULL	allergies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The various factors that can cause a mouthbreathing habit , such as asthma , allergies and enlarged glandular tissue , are discussed in detail .
	manualset3
169090	5	413018	7	NULL	NULL	0	NULL	enlarged glandular tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The various factors that can cause a mouthbreathing habit , such as asthma , allergies and enlarged glandular tissue , are discussed in detail .
	manualset3
169123	1	413019	7	NULL	NULL	0	NULL	varying topography 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The varying topography of the commodities necessitated minor modifications to the method ; for example , analysis of kiwi required that the hair on the surface be shaved prior to swabbing to achieve good recovery .
	manualset3
169124	2	413019	7	NULL	NULL	0	NULL	commodities	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The varying topography of the commodities necessitated minor modifications to the method ; for example , analysis of kiwi required that the hair on the surface be shaved prior to swabbing to achieve good recovery .
	manualset3
169125	3	413019	7	NULL	NULL	0	NULL	minor modifications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The varying topography of the commodities necessitated minor modifications to the method ; for example , analysis of kiwi required that the hair on the surface be shaved prior to swabbing to achieve good recovery .
	manualset3
169126	4	413019	7	NULL	NULL	0	NULL	method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The varying topography of the commodities necessitated minor modifications to the method ; for example , analysis of kiwi required that the hair on the surface be shaved prior to swabbing to achieve good recovery .
	manualset3
169127	5	413019	7	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The varying topography of the commodities necessitated minor modifications to the method ; for example , analysis of kiwi required that the hair on the surface be shaved prior to swabbing to achieve good recovery .
	manualset3
169128	6	413019	7	NULL	NULL	0	NULL	kiwi 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The varying topography of the commodities necessitated minor modifications to the method ; for example , analysis of kiwi required that the hair on the surface be shaved prior to swabbing to achieve good recovery .
	manualset3
169129	7	413019	7	NULL	NULL	0	NULL	 hair	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The varying topography of the commodities necessitated minor modifications to the method ; for example , analysis of kiwi required that the hair on the surface be shaved prior to swabbing to achieve good recovery .
	manualset3
169130	8	413019	7	NULL	NULL	0	NULL	 surface	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The varying topography of the commodities necessitated minor modifications to the method ; for example , analysis of kiwi required that the hair on the surface be shaved prior to swabbing to achieve good recovery .
	manualset3
169131	9	413019	7	NULL	NULL	0	NULL	swabbing 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The varying topography of the commodities necessitated minor modifications to the method ; for example , analysis of kiwi required that the hair on the surface be shaved prior to swabbing to achieve good recovery .
	manualset3
169132	10	413019	7	NULL	NULL	0	NULL	 good recovery	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The varying topography of the commodities necessitated minor modifications to the method ; for example , analysis of kiwi required that the hair on the surface be shaved prior to swabbing to achieve good recovery .
	manualset3
169133	1	413020	7	NULL	NULL	0	NULL	vascular anatomy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The vascular anatomy is evaluated by the combined use of duplex Doppler ultrasonography and computed tomography ( CT ) .
	manualset3
169134	2	413020	7	NULL	NULL	0	NULL	duplex Doppler ultrasonography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The vascular anatomy is evaluated by the combined use of duplex Doppler ultrasonography and computed tomography ( CT ) .
	manualset3
169135	3	413020	7	NULL	NULL	0	NULL	computed tomography ( CT )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The vascular anatomy is evaluated by the combined use of duplex Doppler ultrasonography and computed tomography ( CT ) .
	manualset3
169136	1	413021	7	NULL	NULL	0	NULL	majority	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The vast majority of dormant lymphoma cells are in cell cycle arrest , but there are also residual replicating cells .
	manualset3
169137	2	413021	7	NULL	NULL	0	NULL	dormant lymphoma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The vast majority of dormant lymphoma cells are in cell cycle arrest , but there are also residual replicating cells .
	manualset3
169138	3	413021	7	NULL	NULL	0	NULL	cell cycle arrest	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The vast majority of dormant lymphoma cells are in cell cycle arrest , but there are also residual replicating cells .
	manualset3
169139	4	413021	7	NULL	NULL	0	NULL	residual replicating cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The vast majority of dormant lymphoma cells are in cell cycle arrest , but there are also residual replicating cells .
	manualset3
169140	1	413022	7	NULL	NULL	NULL	NULL	vehicle	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The vehicle , on the other hand , had no effect on baroreflex sensitivity of ovariectomized rats .
	manualset3
169141	2	413022	7	NULL	NULL	0	NULL	baroreflex sensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The vehicle , on the other hand , had no effect on baroreflex sensitivity of ovariectomized rats .
	manualset3
169142	3	413022	7	NULL	NULL	0	NULL	ovariectomized rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The vehicle , on the other hand , had no effect on baroreflex sensitivity of ovariectomized rats .
	manualset3
169143	1	413023	7	NULL	NULL	0	NULL	ventricle extraction method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ventricle extraction method was implemented on the Window platform using C + + , and was validated qualitatively on 30 MRI studies with variable parameters .
	manualset3
169144	2	413023	7	NULL	NULL	0	NULL	 Window platform	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The ventricle extraction method was implemented on the Window platform using C + + , and was validated qualitatively on 30 MRI studies with variable parameters .
	manualset3
169145	3	413023	7	NULL	NULL	0	NULL	C + +	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The ventricle extraction method was implemented on the Window platform using C + + , and was validated qualitatively on 30 MRI studies with variable parameters .
	manualset3
169146	4	413023	7	NULL	NULL	0	NULL	30 MRI studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ventricle extraction method was implemented on the Window platform using C + + , and was validated qualitatively on 30 MRI studies with variable parameters .
	manualset3
169147	5	413023	7	NULL	NULL	0	NULL	variable parameters	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The ventricle extraction method was implemented on the Window platform using C + + , and was validated qualitatively on 30 MRI studies with variable parameters .
	manualset3
169148	1	413024	7	NULL	NULL	0	NULL	verrucous skin lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The verrucous skin lesion was treated successfully with combined topical 5-fluorouracil and vitamin D3 application .
	manualset3
169149	2	413024	7	NULL	NULL	0	NULL	topical 5-fluorouracil	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The verrucous skin lesion was treated successfully with combined topical 5-fluorouracil and vitamin D3 application .
	manualset3
169150	3	413024	7	NULL	NULL	0	NULL	vitamin D3 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The verrucous skin lesion was treated successfully with combined topical 5-fluorouracil and vitamin D3 application .
	manualset3
169151	4	413024	7	NULL	NULL	0	NULL	application	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The verrucous skin lesion was treated successfully with combined topical 5-fluorouracil and vitamin D3 application .
	manualset3
169152	1	413025	7	NULL	NULL	0	NULL	inducible lentiviral RNAi system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The versatile and robust inducible lentiviral RNAi system reported herein can therefore serve as a powerful tool to rapidly reveal tumor cell dependence .
	manualset3
169153	2	413025	7	NULL	NULL	0	NULL	powerful tool 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The versatile and robust inducible lentiviral RNAi system reported herein can therefore serve as a powerful tool to rapidly reveal tumor cell dependence .
	manualset3
169154	3	413025	7	NULL	NULL	0	NULL	tumor cell dependence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The versatile and robust inducible lentiviral RNAi system reported herein can therefore serve as a powerful tool to rapidly reveal tumor cell dependence .
	manualset3
169155	1	413026	7	NULL	NULL	0	NULL	vertebral column	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The vertebral column is the most frequent site of metastatic involvement of the skeleton .
	manualset3
169156	2	413026	7	NULL	NULL	0	NULL	frequent site	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The vertebral column is the most frequent site of metastatic involvement of the skeleton .
	manualset3
169157	3	413026	7	NULL	NULL	0	NULL	metastatic involvement	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The vertebral column is the most frequent site of metastatic involvement of the skeleton .
	manualset3
169158	4	413026	7	NULL	NULL	0	NULL	skeleton	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The vertebral column is the most frequent site of metastatic involvement of the skeleton .
	manualset3
169159	1	413027	7	NULL	NULL	0	NULL	Activation-induced cytidine deaminase ( AID )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation-induced cytidine deaminase ( AID ) induces somatic mutations in various host genes of non-lymphoid tissues , thereby contributing to carcinogenesis .
	manualset3
169160	2	413027	7	NULL	NULL	0	NULL	somatic mutations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation-induced cytidine deaminase ( AID ) induces somatic mutations in various host genes of non-lymphoid tissues , thereby contributing to carcinogenesis .
	manualset3
169161	3	413027	7	NULL	NULL	0	NULL	host genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation-induced cytidine deaminase ( AID ) induces somatic mutations in various host genes of non-lymphoid tissues , thereby contributing to carcinogenesis .
	manualset3
169162	4	413027	7	NULL	NULL	0	NULL	non-lymphoid tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation-induced cytidine deaminase ( AID ) induces somatic mutations in various host genes of non-lymphoid tissues , thereby contributing to carcinogenesis .
	manualset3
169163	5	413027	7	NULL	NULL	0	NULL	carcinogenesis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation-induced cytidine deaminase ( AID ) induces somatic mutations in various host genes of non-lymphoid tissues , thereby contributing to carcinogenesis .
	manualset3
169164	1	413028	7	NULL	NULL	0	NULL	 vertebrate Ena/VASP family 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The vertebrate Ena/VASP family is comprised of three genes : Ena ( Enabled ) , VASP ( Vasodilator Stimulated Phosphoprotein ) , and Evl ( Ena/VASP-Like ) .
	manualset3
169165	2	413028	7	NULL	NULL	0	NULL	three genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The vertebrate Ena/VASP family is comprised of three genes : Ena ( Enabled ) , VASP ( Vasodilator Stimulated Phosphoprotein ) , and Evl ( Ena/VASP-Like ) .
	manualset3
169166	3	413028	7	NULL	NULL	0	NULL	Ena ( Enabled ) 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The vertebrate Ena/VASP family is comprised of three genes : Ena ( Enabled ) , VASP ( Vasodilator Stimulated Phosphoprotein ) , and Evl ( Ena/VASP-Like ) .
	manualset3
169167	4	413028	7	NULL	NULL	0	NULL	VASP ( Vasodilator Stimulated Phosphoprotein )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The vertebrate Ena/VASP family is comprised of three genes : Ena ( Enabled ) , VASP ( Vasodilator Stimulated Phosphoprotein ) , and Evl ( Ena/VASP-Like ) .
	manualset3
169168	5	413028	7	NULL	NULL	0	NULL	Evl ( Ena/VASP-Like )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The vertebrate Ena/VASP family is comprised of three genes : Ena ( Enabled ) , VASP ( Vasodilator Stimulated Phosphoprotein ) , and Evl ( Ena/VASP-Like ) .
	manualset3
169169	1	413029	7	NULL	NULL	0	NULL	vertical distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The vertical distribution of LAS in the water column was not homogeneous , in contrast to that presented by the SPC homologs .
	manualset3
169170	2	413029	7	NULL	NULL	0	NULL	LAS	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The vertical distribution of LAS in the water column was not homogeneous , in contrast to that presented by the SPC homologs .
	manualset3
169171	3	413029	7	NULL	NULL	NULL	NULL	water column	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The vertical distribution of LAS in the water column was not homogeneous , in contrast to that presented by the SPC homologs .
	manualset3
169172	4	413029	7	NULL	NULL	0	NULL	SPC homologs	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The vertical distribution of LAS in the water column was not homogeneous , in contrast to that presented by the SPC homologs .
	manualset3
169173	1	413030	7	NULL	NULL	NULL	NULL	 very low reactivity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The very low reactivity of ( Fe ( III ) ( tpfpp ) ( OH ) ( OOH ) ) towards organic substrates implied that the ferric hydroperoxo intermediate must be a very sluggish oxidant compared with the iron ( IV ) - oxo porphyrin - cation radical intermediate in the catalytic oxygenation reactions of cytochrome P450 .
	manualset3
169174	2	413030	7	NULL	NULL	0	NULL	( Fe ( III ) ( tpfpp ) ( OH ) ( OOH ) )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The very low reactivity of ( Fe ( III ) ( tpfpp ) ( OH ) ( OOH ) ) towards organic substrates implied that the ferric hydroperoxo intermediate must be a very sluggish oxidant compared with the iron ( IV ) - oxo porphyrin - cation radical intermediate in the catalytic oxygenation reactions of cytochrome P450 .
	manualset3
169175	3	413030	7	NULL	NULL	NULL	NULL	organic substrates	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The very low reactivity of ( Fe ( III ) ( tpfpp ) ( OH ) ( OOH ) ) towards organic substrates implied that the ferric hydroperoxo intermediate must be a very sluggish oxidant compared with the iron ( IV ) - oxo porphyrin - cation radical intermediate in the catalytic oxygenation reactions of cytochrome P450 .
	manualset3
169176	4	413030	7	NULL	NULL	0	NULL	ferric hydroperoxo intermediate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The very low reactivity of ( Fe ( III ) ( tpfpp ) ( OH ) ( OOH ) ) towards organic substrates implied that the ferric hydroperoxo intermediate must be a very sluggish oxidant compared with the iron ( IV ) - oxo porphyrin - cation radical intermediate in the catalytic oxygenation reactions of cytochrome P450 .
	manualset3
169177	5	413030	7	NULL	NULL	0	NULL	sluggish oxidant	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The very low reactivity of ( Fe ( III ) ( tpfpp ) ( OH ) ( OOH ) ) towards organic substrates implied that the ferric hydroperoxo intermediate must be a very sluggish oxidant compared with the iron ( IV ) - oxo porphyrin - cation radical intermediate in the catalytic oxygenation reactions of cytochrome P450 .
	manualset3
169178	6	413030	7	NULL	NULL	0	NULL	iron ( IV ) - oxo porphyrin - cation radical intermediate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The very low reactivity of ( Fe ( III ) ( tpfpp ) ( OH ) ( OOH ) ) towards organic substrates implied that the ferric hydroperoxo intermediate must be a very sluggish oxidant compared with the iron ( IV ) - oxo porphyrin - cation radical intermediate in the catalytic oxygenation reactions of cytochrome P450 .
	manualset3
169179	7	413030	7	NULL	NULL	NULL	NULL	catalytic oxygenation reactions	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The very low reactivity of ( Fe ( III ) ( tpfpp ) ( OH ) ( OOH ) ) towards organic substrates implied that the ferric hydroperoxo intermediate must be a very sluggish oxidant compared with the iron ( IV ) - oxo porphyrin - cation radical intermediate in the catalytic oxygenation reactions of cytochrome P450 .
	manualset3
169180	8	413030	7	NULL	NULL	0	NULL	cytochrome P450	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The very low reactivity of ( Fe ( III ) ( tpfpp ) ( OH ) ( OOH ) ) towards organic substrates implied that the ferric hydroperoxo intermediate must be a very sluggish oxidant compared with the iron ( IV ) - oxo porphyrin - cation radical intermediate in the catalytic oxygenation reactions of cytochrome P450 .
	manualset3
169732	1	413031	7	NULL	NULL	0	NULL	viral nucleoproteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The viral nucleoproteins are central to transcription , replication , and packaging of the RNA genome .
	manualset3
169733	2	413031	7	NULL	NULL	0	NULL	transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The viral nucleoproteins are central to transcription , replication , and packaging of the RNA genome .
	manualset3
169734	3	413031	7	NULL	NULL	0	NULL	replication	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The viral nucleoproteins are central to transcription , replication , and packaging of the RNA genome .
	manualset3
169735	4	413031	7	NULL	NULL	0	NULL	packaging 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The viral nucleoproteins are central to transcription , replication , and packaging of the RNA genome .
	manualset3
169736	5	413031	7	NULL	NULL	0	NULL	RNA genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The viral nucleoproteins are central to transcription , replication , and packaging of the RNA genome .
	manualset3
169737	1	413032	7	NULL	NULL	0	NULL	virulence profiles	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The virulence profiles of most non-O157 Shiga toxin ( Stx ) - producing Escherichia coli ( STEC ) are unknown .
	manualset3
169738	2	413032	7	NULL	NULL	0	NULL	non-O157 Shiga toxin ( Stx ) - producing Escherichia coli ( STEC )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The virulence profiles of most non-O157 Shiga toxin ( Stx ) - producing Escherichia coli ( STEC ) are unknown .
	manualset3
169739	1	413033	7	NULL	NULL	0	NULL	virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The virus responsible for herpes is a double-stranded DNA virus named Herpes simplex virus ( HSV ) .
	manualset3
169740	2	413033	7	NULL	NULL	0	NULL	herpes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The virus responsible for herpes is a double-stranded DNA virus named Herpes simplex virus ( HSV ) .
	manualset3
169741	3	413033	7	NULL	NULL	0	NULL	 double-stranded DNA virus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The virus responsible for herpes is a double-stranded DNA virus named Herpes simplex virus ( HSV ) .
	manualset3
169742	4	413033	7	NULL	NULL	0	NULL	Herpes simplex virus ( HSV )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The virus responsible for herpes is a double-stranded DNA virus named Herpes simplex virus ( HSV ) .
	manualset3
169743	1	413034	7	NULL	NULL	0	NULL	virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The virus was responsible for a recent hemorrhagic fever outbreak in Uganda with an approximate 30 % case fatality rate .
	manualset3
169744	2	413034	7	NULL	NULL	0	NULL	hemorrhagic fever outbreak	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The virus was responsible for a recent hemorrhagic fever outbreak in Uganda with an approximate 30 % case fatality rate .
	manualset3
169745	3	413034	7	NULL	NULL	0	NULL	Uganda	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The virus was responsible for a recent hemorrhagic fever outbreak in Uganda with an approximate 30 % case fatality rate .
	manualset3
169746	4	413034	7	NULL	NULL	0	NULL	30 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The virus was responsible for a recent hemorrhagic fever outbreak in Uganda with an approximate 30 % case fatality rate .
	manualset3
169747	5	413034	7	NULL	NULL	0	NULL	case fatality rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The virus was responsible for a recent hemorrhagic fever outbreak in Uganda with an approximate 30 % case fatality rate .
	manualset3
169748	1	413035	7	NULL	NULL	0	NULL	 viruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The viruses contain a single-stranded RNA genome , but appreciable amounts of ribosomal-like RNA and 4-6S RNA of host cell origin have been detected .
	manualset3
169749	2	413035	7	NULL	NULL	0	NULL	single-stranded RNA genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The viruses contain a single-stranded RNA genome , but appreciable amounts of ribosomal-like RNA and 4-6S RNA of host cell origin have been detected .
	manualset3
169750	3	413035	7	NULL	NULL	0	NULL	amounts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The viruses contain a single-stranded RNA genome , but appreciable amounts of ribosomal-like RNA and 4-6S RNA of host cell origin have been detected .
	manualset3
169751	4	413035	7	NULL	NULL	0	NULL	 ribosomal-like RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The viruses contain a single-stranded RNA genome , but appreciable amounts of ribosomal-like RNA and 4-6S RNA of host cell origin have been detected .
	manualset3
169752	5	413035	7	NULL	NULL	0	NULL	4-6S RNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The viruses contain a single-stranded RNA genome , but appreciable amounts of ribosomal-like RNA and 4-6S RNA of host cell origin have been detected .
	manualset3
169753	6	413035	7	NULL	NULL	0	NULL	host cell origin	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The viruses contain a single-stranded RNA genome , but appreciable amounts of ribosomal-like RNA and 4-6S RNA of host cell origin have been detected .
	manualset3
169754	1	413036	7	NULL	NULL	NULL	NULL	visual or morphometric assessment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The visual or morphometric assessment of lateral DXA spine images may have a potential role for use as a prescreening tool , excluding normal subjects prior to performing conventional radiographs .
	manualset3
169755	2	413036	7	NULL	NULL	0	NULL	lateral DXA spine images	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The visual or morphometric assessment of lateral DXA spine images may have a potential role for use as a prescreening tool , excluding normal subjects prior to performing conventional radiographs .
	manualset3
169756	3	413036	7	NULL	NULL	0	NULL	potential role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The visual or morphometric assessment of lateral DXA spine images may have a potential role for use as a prescreening tool , excluding normal subjects prior to performing conventional radiographs .
	manualset3
169757	4	413036	7	NULL	NULL	0	NULL	prescreening tool	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The visual or morphometric assessment of lateral DXA spine images may have a potential role for use as a prescreening tool , excluding normal subjects prior to performing conventional radiographs .
	manualset3
169758	5	413036	7	NULL	NULL	0	NULL	normal subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The visual or morphometric assessment of lateral DXA spine images may have a potential role for use as a prescreening tool , excluding normal subjects prior to performing conventional radiographs .
	manualset3
169759	6	413036	7	NULL	NULL	0	NULL	conventional radiographs	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The visual or morphometric assessment of lateral DXA spine images may have a potential role for use as a prescreening tool , excluding normal subjects prior to performing conventional radiographs .
	manualset3
169760	1	413037	7	NULL	NULL	NULL	NULL	voltammetric behaviors	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The voltammetric behaviors of trazodone using a platinum electrode in stationary or rotating conditions and its determination in tablets by DP rotating electrodes are described in this study .
	manualset3
169793	2	413037	7	NULL	NULL	0	NULL	trazodone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The voltammetric behaviors of trazodone using a platinum electrode in stationary or rotating conditions and its determination in tablets by DP rotating electrodes are described in this study .
	manualset3
169794	3	413037	7	NULL	NULL	0	NULL	platinum electrode	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The voltammetric behaviors of trazodone using a platinum electrode in stationary or rotating conditions and its determination in tablets by DP rotating electrodes are described in this study .
	manualset3
169795	4	413037	7	NULL	NULL	0	NULL	stationary condition	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The voltammetric behaviors of trazodone using a platinum electrode in stationary or rotating conditions and its determination in tablets by DP rotating electrodes are described in this study .
	manualset3
169796	5	413037	7	NULL	NULL	0	NULL	rotating conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The voltammetric behaviors of trazodone using a platinum electrode in stationary or rotating conditions and its determination in tablets by DP rotating electrodes are described in this study .
	manualset3
169797	6	413037	7	NULL	NULL	0	NULL	determination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The voltammetric behaviors of trazodone using a platinum electrode in stationary or rotating conditions and its determination in tablets by DP rotating electrodes are described in this study .
	manualset3
169798	7	413037	7	NULL	NULL	0	NULL	tablets	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The voltammetric behaviors of trazodone using a platinum electrode in stationary or rotating conditions and its determination in tablets by DP rotating electrodes are described in this study .
	manualset3
169799	8	413037	7	NULL	NULL	0	NULL	DP rotating electrodes	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The voltammetric behaviors of trazodone using a platinum electrode in stationary or rotating conditions and its determination in tablets by DP rotating electrodes are described in this study .
	manualset3
169800	9	413037	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The voltammetric behaviors of trazodone using a platinum electrode in stationary or rotating conditions and its determination in tablets by DP rotating electrodes are described in this study .
	manualset3
169801	1	413038	7	NULL	NULL	0	NULL	volume of bone	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The volume of bone in the gap was increased by 16 % in rhTGF-beta1-stimulated TCP-coated implants , but this difference was not significant .
	manualset3
169802	2	413038	7	NULL	NULL	0	NULL	gap	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The volume of bone in the gap was increased by 16 % in rhTGF-beta1-stimulated TCP-coated implants , but this difference was not significant .
	manualset3
169803	3	413038	7	NULL	NULL	0	NULL	16 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The volume of bone in the gap was increased by 16 % in rhTGF-beta1-stimulated TCP-coated implants , but this difference was not significant .
	manualset3
169804	4	413038	7	NULL	NULL	0	NULL	rhTGF-beta1-stimulated TCP-coated implants	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The volume of bone in the gap was increased by 16 % in rhTGF-beta1-stimulated TCP-coated implants , but this difference was not significant .
	manualset3
169805	5	413038	7	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The volume of bone in the gap was increased by 16 % in rhTGF-beta1-stimulated TCP-coated implants , but this difference was not significant .
	manualset3
169806	1	413039	7	NULL	NULL	0	NULL	volume	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The volume of distribution of sodium thiosulphate in sheep .
	manualset3
169807	2	413039	7	NULL	NULL	0	NULL	distribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The volume of distribution of sodium thiosulphate in sheep .
	manualset3
169808	3	413039	7	NULL	NULL	0	NULL	sodium thiosulphate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The volume of distribution of sodium thiosulphate in sheep .
	manualset3
169809	4	413039	7	NULL	NULL	0	NULL	 sheep	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The volume of distribution of sodium thiosulphate in sheep .
	manualset3
169810	1	413040	7	NULL	NULL	0	NULL	water mol-ecules	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The water mol-ecules occupy voids between the chains .
	manualset3
169811	2	413040	7	NULL	NULL	0	NULL	voids	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The water mol-ecules occupy voids between the chains .
	manualset3
169812	3	413040	7	NULL	NULL	0	NULL	chains	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The water mol-ecules occupy voids between the chains .
	manualset3
169813	1	413041	7	NULL	NULL	0	NULL	 weaned ( W ) group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The weaned ( W ) group was finished on concentrate and hay , whereas the non-weaned ( NW ) group was finished on concentrate and hay and it continued suckling until slaughter .
	manualset3
169814	2	413041	7	NULL	NULL	NULL	NULL	concentrate	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The weaned ( W ) group was finished on concentrate and hay , whereas the non-weaned ( NW ) group was finished on concentrate and hay and it continued suckling until slaughter .
	manualset3
169815	3	413041	7	NULL	NULL	0	NULL	hay	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The weaned ( W ) group was finished on concentrate and hay , whereas the non-weaned ( NW ) group was finished on concentrate and hay and it continued suckling until slaughter .
	manualset3
169816	4	413041	7	NULL	NULL	0	NULL	non-weaned ( NW ) group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The weaned ( W ) group was finished on concentrate and hay , whereas the non-weaned ( NW ) group was finished on concentrate and hay and it continued suckling until slaughter .
	manualset3
169817	5	413041	7	NULL	NULL	NULL	NULL	concentrate	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The weaned ( W ) group was finished on concentrate and hay , whereas the non-weaned ( NW ) group was finished on concentrate and hay and it continued suckling until slaughter .
	manualset3
169818	6	413041	7	NULL	NULL	0	NULL	hay	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The weaned ( W ) group was finished on concentrate and hay , whereas the non-weaned ( NW ) group was finished on concentrate and hay and it continued suckling until slaughter .
	manualset3
169819	7	413041	7	NULL	NULL	0	NULL	suckling	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The weaned ( W ) group was finished on concentrate and hay , whereas the non-weaned ( NW ) group was finished on concentrate and hay and it continued suckling until slaughter .
	manualset3
169820	8	413041	7	NULL	NULL	0	NULL	slaughter	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The weaned ( W ) group was finished on concentrate and hay , whereas the non-weaned ( NW ) group was finished on concentrate and hay and it continued suckling until slaughter .
	manualset3
169821	1	413042	7	NULL	NULL	0	NULL	 wear vectors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The wear vectors in 41 retrieved implants from a single manufacturer were measured with use of the shadowgraph technique , and the spatial orientation of each implant was calculated from serial anteroposterior pelvic radiographs .
	manualset3
169822	2	413042	7	NULL	NULL	0	NULL	 41 retrieved implants	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The wear vectors in 41 retrieved implants from a single manufacturer were measured with use of the shadowgraph technique , and the spatial orientation of each implant was calculated from serial anteroposterior pelvic radiographs .
	manualset3
169823	3	413042	7	NULL	NULL	NULL	NULL	 single manufacturer	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The wear vectors in 41 retrieved implants from a single manufacturer were measured with use of the shadowgraph technique , and the spatial orientation of each implant was calculated from serial anteroposterior pelvic radiographs .
	manualset3
169824	4	413042	7	NULL	NULL	0	NULL	shadowgraph technique	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The wear vectors in 41 retrieved implants from a single manufacturer were measured with use of the shadowgraph technique , and the spatial orientation of each implant was calculated from serial anteroposterior pelvic radiographs .
	manualset3
169825	5	413042	7	NULL	NULL	0	NULL	spatial orientation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The wear vectors in 41 retrieved implants from a single manufacturer were measured with use of the shadowgraph technique , and the spatial orientation of each implant was calculated from serial anteroposterior pelvic radiographs .
	manualset3
169826	6	413042	7	NULL	NULL	0	NULL	 implant	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The wear vectors in 41 retrieved implants from a single manufacturer were measured with use of the shadowgraph technique , and the spatial orientation of each implant was calculated from serial anteroposterior pelvic radiographs .
	manualset3
169827	7	413042	7	NULL	NULL	0	NULL	serial anteroposterior pelvic radiographs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The wear vectors in 41 retrieved implants from a single manufacturer were measured with use of the shadowgraph technique , and the spatial orientation of each implant was calculated from serial anteroposterior pelvic radiographs .
	manualset3
169828	1	413043	7	NULL	NULL	0	NULL	whole	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The whole of these results demonstrated that , in this model , SIV establishes a persistent state of infection of astrocytes , that viral replication can be reactivated by cytokines and moreover suggest strongly an in vivo infection of astrocytes in the brain of these infected macaques .
	manualset3
169829	2	413043	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The whole of these results demonstrated that , in this model , SIV establishes a persistent state of infection of astrocytes , that viral replication can be reactivated by cytokines and moreover suggest strongly an in vivo infection of astrocytes in the brain of these infected macaques .
	manualset3
169830	3	413043	7	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The whole of these results demonstrated that , in this model , SIV establishes a persistent state of infection of astrocytes , that viral replication can be reactivated by cytokines and moreover suggest strongly an in vivo infection of astrocytes in the brain of these infected macaques .
	manualset3
169831	4	413043	7	NULL	NULL	0	NULL	SIV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The whole of these results demonstrated that , in this model , SIV establishes a persistent state of infection of astrocytes , that viral replication can be reactivated by cytokines and moreover suggest strongly an in vivo infection of astrocytes in the brain of these infected macaques .
	manualset3
169832	5	413043	7	NULL	NULL	0	NULL	persistent state	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The whole of these results demonstrated that , in this model , SIV establishes a persistent state of infection of astrocytes , that viral replication can be reactivated by cytokines and moreover suggest strongly an in vivo infection of astrocytes in the brain of these infected macaques .
	manualset3
169833	6	413043	7	NULL	NULL	NULL	NULL	infection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The whole of these results demonstrated that , in this model , SIV establishes a persistent state of infection of astrocytes , that viral replication can be reactivated by cytokines and moreover suggest strongly an in vivo infection of astrocytes in the brain of these infected macaques .
	manualset3
169834	7	413043	7	NULL	NULL	0	NULL	astrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The whole of these results demonstrated that , in this model , SIV establishes a persistent state of infection of astrocytes , that viral replication can be reactivated by cytokines and moreover suggest strongly an in vivo infection of astrocytes in the brain of these infected macaques .
	manualset3
169835	8	413043	7	NULL	NULL	0	NULL	viral replication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The whole of these results demonstrated that , in this model , SIV establishes a persistent state of infection of astrocytes , that viral replication can be reactivated by cytokines and moreover suggest strongly an in vivo infection of astrocytes in the brain of these infected macaques .
	manualset3
169836	9	413043	7	NULL	NULL	0	NULL	cytokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The whole of these results demonstrated that , in this model , SIV establishes a persistent state of infection of astrocytes , that viral replication can be reactivated by cytokines and moreover suggest strongly an in vivo infection of astrocytes in the brain of these infected macaques .
	manualset3
169837	10	413043	7	NULL	NULL	0	NULL	in vivo infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The whole of these results demonstrated that , in this model , SIV establishes a persistent state of infection of astrocytes , that viral replication can be reactivated by cytokines and moreover suggest strongly an in vivo infection of astrocytes in the brain of these infected macaques .
	manualset3
169838	11	413043	7	NULL	NULL	0	NULL	astrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The whole of these results demonstrated that , in this model , SIV establishes a persistent state of infection of astrocytes , that viral replication can be reactivated by cytokines and moreover suggest strongly an in vivo infection of astrocytes in the brain of these infected macaques .
	manualset3
169839	12	413043	7	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The whole of these results demonstrated that , in this model , SIV establishes a persistent state of infection of astrocytes , that viral replication can be reactivated by cytokines and moreover suggest strongly an in vivo infection of astrocytes in the brain of these infected macaques .
	manualset3
169840	13	413043	7	NULL	NULL	0	NULL	infected macaques	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The whole of these results demonstrated that , in this model , SIV establishes a persistent state of infection of astrocytes , that viral replication can be reactivated by cytokines and moreover suggest strongly an in vivo infection of astrocytes in the brain of these infected macaques .
	manualset3
169841	1	413044	7	NULL	NULL	0	NULL	wide range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The wide range of results in the ratio of skew-miniature endplate potential to bell-miniature endplate potential classes is discussed in regards to the quantal hypothesis which is based on a single class of immutable amounts of transmitter ; and , a hypothesis based on a dynamical process that meters transmitter in subunit amounts to control miniature endplate potential size and class during release .
	manualset3
169842	2	413044	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The wide range of results in the ratio of skew-miniature endplate potential to bell-miniature endplate potential classes is discussed in regards to the quantal hypothesis which is based on a single class of immutable amounts of transmitter ; and , a hypothesis based on a dynamical process that meters transmitter in subunit amounts to control miniature endplate potential size and class during release .
	manualset3
169843	3	413044	7	NULL	NULL	0	NULL	 ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The wide range of results in the ratio of skew-miniature endplate potential to bell-miniature endplate potential classes is discussed in regards to the quantal hypothesis which is based on a single class of immutable amounts of transmitter ; and , a hypothesis based on a dynamical process that meters transmitter in subunit amounts to control miniature endplate potential size and class during release .
	manualset3
169844	4	413044	7	NULL	NULL	0	NULL	skew-miniature endplate potential	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The wide range of results in the ratio of skew-miniature endplate potential to bell-miniature endplate potential classes is discussed in regards to the quantal hypothesis which is based on a single class of immutable amounts of transmitter ; and , a hypothesis based on a dynamical process that meters transmitter in subunit amounts to control miniature endplate potential size and class during release .
	manualset3
169845	5	413044	7	NULL	NULL	0	NULL	bell-miniature endplate potential classes 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The wide range of results in the ratio of skew-miniature endplate potential to bell-miniature endplate potential classes is discussed in regards to the quantal hypothesis which is based on a single class of immutable amounts of transmitter ; and , a hypothesis based on a dynamical process that meters transmitter in subunit amounts to control miniature endplate potential size and class during release .
	manualset3
169846	6	413044	7	NULL	NULL	0	NULL	quantal hypothesis 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The wide range of results in the ratio of skew-miniature endplate potential to bell-miniature endplate potential classes is discussed in regards to the quantal hypothesis which is based on a single class of immutable amounts of transmitter ; and , a hypothesis based on a dynamical process that meters transmitter in subunit amounts to control miniature endplate potential size and class during release .
	manualset3
169847	7	413044	7	NULL	NULL	0	NULL	single class	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The wide range of results in the ratio of skew-miniature endplate potential to bell-miniature endplate potential classes is discussed in regards to the quantal hypothesis which is based on a single class of immutable amounts of transmitter ; and , a hypothesis based on a dynamical process that meters transmitter in subunit amounts to control miniature endplate potential size and class during release .
	manualset3
169848	8	413044	7	NULL	NULL	0	NULL	immutable amounts 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The wide range of results in the ratio of skew-miniature endplate potential to bell-miniature endplate potential classes is discussed in regards to the quantal hypothesis which is based on a single class of immutable amounts of transmitter ; and , a hypothesis based on a dynamical process that meters transmitter in subunit amounts to control miniature endplate potential size and class during release .
	manualset3
169849	9	413044	7	NULL	NULL	0	NULL	 transmitter	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The wide range of results in the ratio of skew-miniature endplate potential to bell-miniature endplate potential classes is discussed in regards to the quantal hypothesis which is based on a single class of immutable amounts of transmitter ; and , a hypothesis based on a dynamical process that meters transmitter in subunit amounts to control miniature endplate potential size and class during release .
	manualset3
169850	10	413044	7	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The wide range of results in the ratio of skew-miniature endplate potential to bell-miniature endplate potential classes is discussed in regards to the quantal hypothesis which is based on a single class of immutable amounts of transmitter ; and , a hypothesis based on a dynamical process that meters transmitter in subunit amounts to control miniature endplate potential size and class during release .
	manualset3
169851	11	413044	7	NULL	NULL	0	NULL	 dynamical process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The wide range of results in the ratio of skew-miniature endplate potential to bell-miniature endplate potential classes is discussed in regards to the quantal hypothesis which is based on a single class of immutable amounts of transmitter ; and , a hypothesis based on a dynamical process that meters transmitter in subunit amounts to control miniature endplate potential size and class during release .
	manualset3
169852	12	413044	7	NULL	NULL	0	NULL	 transmitter 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The wide range of results in the ratio of skew-miniature endplate potential to bell-miniature endplate potential classes is discussed in regards to the quantal hypothesis which is based on a single class of immutable amounts of transmitter ; and , a hypothesis based on a dynamical process that meters transmitter in subunit amounts to control miniature endplate potential size and class during release .
	manualset3
169853	13	413044	7	NULL	NULL	0	NULL	subunit amounts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The wide range of results in the ratio of skew-miniature endplate potential to bell-miniature endplate potential classes is discussed in regards to the quantal hypothesis which is based on a single class of immutable amounts of transmitter ; and , a hypothesis based on a dynamical process that meters transmitter in subunit amounts to control miniature endplate potential size and class during release .
	manualset3
169854	14	413044	7	NULL	NULL	0	NULL	miniature endplate potential size 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The wide range of results in the ratio of skew-miniature endplate potential to bell-miniature endplate potential classes is discussed in regards to the quantal hypothesis which is based on a single class of immutable amounts of transmitter ; and , a hypothesis based on a dynamical process that meters transmitter in subunit amounts to control miniature endplate potential size and class during release .
	manualset3
169855	15	413044	7	NULL	NULL	0	NULL	 class	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The wide range of results in the ratio of skew-miniature endplate potential to bell-miniature endplate potential classes is discussed in regards to the quantal hypothesis which is based on a single class of immutable amounts of transmitter ; and , a hypothesis based on a dynamical process that meters transmitter in subunit amounts to control miniature endplate potential size and class during release .
	manualset3
169856	16	413044	7	NULL	NULL	0	NULL	release	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The wide range of results in the ratio of skew-miniature endplate potential to bell-miniature endplate potential classes is discussed in regards to the quantal hypothesis which is based on a single class of immutable amounts of transmitter ; and , a hypothesis based on a dynamical process that meters transmitter in subunit amounts to control miniature endplate potential size and class during release .
	manualset3
169857	1	413045	7	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The widely accepted association between aberrant methylation at specific imprinted loci and distinct imprinting disorders has recently been brought into question by the identification of methylation defects at multiple loci ( multilocus methylation defect ( MLMD ) ) .
	manualset3
169858	2	413045	7	NULL	NULL	0	NULL	aberrant methylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The widely accepted association between aberrant methylation at specific imprinted loci and distinct imprinting disorders has recently been brought into question by the identification of methylation defects at multiple loci ( multilocus methylation defect ( MLMD ) ) .
	manualset3
169859	3	413045	7	NULL	NULL	0	NULL	 imprinted loci	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The widely accepted association between aberrant methylation at specific imprinted loci and distinct imprinting disorders has recently been brought into question by the identification of methylation defects at multiple loci ( multilocus methylation defect ( MLMD ) ) .
	manualset3
169860	4	413045	7	NULL	NULL	0	NULL	imprinting disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The widely accepted association between aberrant methylation at specific imprinted loci and distinct imprinting disorders has recently been brought into question by the identification of methylation defects at multiple loci ( multilocus methylation defect ( MLMD ) ) .
	manualset3
169861	5	413045	7	NULL	NULL	0	NULL	question 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The widely accepted association between aberrant methylation at specific imprinted loci and distinct imprinting disorders has recently been brought into question by the identification of methylation defects at multiple loci ( multilocus methylation defect ( MLMD ) ) .
	manualset3
169862	6	413045	7	NULL	NULL	0	NULL	 identification	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The widely accepted association between aberrant methylation at specific imprinted loci and distinct imprinting disorders has recently been brought into question by the identification of methylation defects at multiple loci ( multilocus methylation defect ( MLMD ) ) .
	manualset3
169863	7	413045	7	NULL	NULL	0	NULL	methylation defects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The widely accepted association between aberrant methylation at specific imprinted loci and distinct imprinting disorders has recently been brought into question by the identification of methylation defects at multiple loci ( multilocus methylation defect ( MLMD ) ) .
	manualset3
169864	8	413045	7	NULL	NULL	0	NULL	multiple loci 	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The widely accepted association between aberrant methylation at specific imprinted loci and distinct imprinting disorders has recently been brought into question by the identification of methylation defects at multiple loci ( multilocus methylation defect ( MLMD ) ) .
	manualset3
169865	9	413045	7	NULL	NULL	0	NULL	multilocus methylation defect ( MLMD ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The widely accepted association between aberrant methylation at specific imprinted loci and distinct imprinting disorders has recently been brought into question by the identification of methylation defects at multiple loci ( multilocus methylation defect ( MLMD ) ) .
	manualset3
169866	1	413046	7	NULL	NULL	0	NULL	Activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation in culture of T lymphoma cells with lipopolysaccharide-stimulated macrophages induces the expression of IL-1alpha .
	manualset3
169868	3	413046	7	NULL	NULL	NULL	NULL	culture of T lymphoma cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Activation in culture of T lymphoma cells with lipopolysaccharide-stimulated macrophages induces the expression of IL-1alpha .
	manualset3
169869	4	413046	7	NULL	NULL	0	NULL	lipopolysaccharide-stimulated macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation in culture of T lymphoma cells with lipopolysaccharide-stimulated macrophages induces the expression of IL-1alpha .
	manualset3
169870	5	413046	7	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation in culture of T lymphoma cells with lipopolysaccharide-stimulated macrophages induces the expression of IL-1alpha .
	manualset3
169871	6	413046	7	NULL	NULL	0	NULL	IL-1alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation in culture of T lymphoma cells with lipopolysaccharide-stimulated macrophages induces the expression of IL-1alpha .
	manualset3
169872	1	413047	7	NULL	NULL	0	NULL	application	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The widespread application of day surgery and video-assisted surgery substantiates this evolution of surgery in Italy .
	manualset3
169873	2	413047	7	NULL	NULL	0	NULL	day surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The widespread application of day surgery and video-assisted surgery substantiates this evolution of surgery in Italy .
	manualset3
169874	3	413047	7	NULL	NULL	0	NULL	video-assisted surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The widespread application of day surgery and video-assisted surgery substantiates this evolution of surgery in Italy .
	manualset3
169875	4	413047	7	NULL	NULL	0	NULL	evolution	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The widespread application of day surgery and video-assisted surgery substantiates this evolution of surgery in Italy .
	manualset3
169876	5	413047	7	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The widespread application of day surgery and video-assisted surgery substantiates this evolution of surgery in Italy .
	manualset3
169877	6	413047	7	NULL	NULL	0	NULL	Italy	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The widespread application of day surgery and video-assisted surgery substantiates this evolution of surgery in Italy .
	manualset3
169878	1	413048	7	NULL	NULL	0	NULL	 role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The widespread role of somatostatin ( SRIF ) as a mediator of function in the brain and gut has stimulated interest in it mechanism of action .
	manualset3
169879	2	413048	7	NULL	NULL	0	NULL	 somatostatin ( SRIF )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The widespread role of somatostatin ( SRIF ) as a mediator of function in the brain and gut has stimulated interest in it mechanism of action .
	manualset3
169880	3	413048	7	NULL	NULL	0	NULL	mediator	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The widespread role of somatostatin ( SRIF ) as a mediator of function in the brain and gut has stimulated interest in it mechanism of action .
	manualset3
169881	4	413048	7	NULL	NULL	0	NULL	function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The widespread role of somatostatin ( SRIF ) as a mediator of function in the brain and gut has stimulated interest in it mechanism of action .
	manualset3
169882	5	413048	7	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The widespread role of somatostatin ( SRIF ) as a mediator of function in the brain and gut has stimulated interest in it mechanism of action .
	manualset3
169883	6	413048	7	NULL	NULL	0	NULL	gut 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The widespread role of somatostatin ( SRIF ) as a mediator of function in the brain and gut has stimulated interest in it mechanism of action .
	manualset3
169884	7	413048	7	NULL	NULL	NULL	NULL	 interest	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The widespread role of somatostatin ( SRIF ) as a mediator of function in the brain and gut has stimulated interest in it mechanism of action .
	manualset3
169885	8	413048	7	NULL	NULL	0	NULL	mechanism of action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The widespread role of somatostatin ( SRIF ) as a mediator of function in the brain and gut has stimulated interest in it mechanism of action .
	manualset3
169886	1	413049	7	NULL	NULL	0	NULL	wife	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The wife of the non-present husband has the same personality traits but does not expect help from her husband in the crisis situation and therefore does not request his presence .
	manualset3
169887	2	413049	7	NULL	NULL	0	NULL	non-present husband 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The wife of the non-present husband has the same personality traits but does not expect help from her husband in the crisis situation and therefore does not request his presence .
	manualset3
169888	3	413049	7	NULL	NULL	0	NULL	personality traits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The wife of the non-present husband has the same personality traits but does not expect help from her husband in the crisis situation and therefore does not request his presence .
	manualset3
169889	4	413049	7	NULL	NULL	0	NULL	 help	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The wife of the non-present husband has the same personality traits but does not expect help from her husband in the crisis situation and therefore does not request his presence .
	manualset3
169890	5	413049	7	NULL	NULL	0	NULL	husband	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The wife of the non-present husband has the same personality traits but does not expect help from her husband in the crisis situation and therefore does not request his presence .
	manualset3
169891	6	413049	7	NULL	NULL	0	NULL	crisis situation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The wife of the non-present husband has the same personality traits but does not expect help from her husband in the crisis situation and therefore does not request his presence .
	manualset3
169892	1	413050	7	NULL	NULL	0	NULL	window	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The window lies between two noise sources , a low-frequency one attributed to turbulence , and a high-frequency one ( 200-500 Hz ) attributed to bubble noise from water breaking the surface .
	manualset3
169893	2	413050	7	NULL	NULL	0	NULL	two noise sources	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The window lies between two noise sources , a low-frequency one attributed to turbulence , and a high-frequency one ( 200-500 Hz ) attributed to bubble noise from water breaking the surface .
	manualset3
169894	3	413050	7	NULL	NULL	0	NULL	low-frequency 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The window lies between two noise sources , a low-frequency one attributed to turbulence , and a high-frequency one ( 200-500 Hz ) attributed to bubble noise from water breaking the surface .
	manualset3
169895	4	413050	7	NULL	NULL	0	NULL	turbulence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The window lies between two noise sources , a low-frequency one attributed to turbulence , and a high-frequency one ( 200-500 Hz ) attributed to bubble noise from water breaking the surface .
	manualset3
169896	5	413050	7	NULL	NULL	0	NULL	high-frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The window lies between two noise sources , a low-frequency one attributed to turbulence , and a high-frequency one ( 200-500 Hz ) attributed to bubble noise from water breaking the surface .
	manualset3
169897	6	413050	7	NULL	NULL	0	NULL	200-500 Hz	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The window lies between two noise sources , a low-frequency one attributed to turbulence , and a high-frequency one ( 200-500 Hz ) attributed to bubble noise from water breaking the surface .
	manualset3
169898	7	413050	7	NULL	NULL	0	NULL	bubble noise	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The window lies between two noise sources , a low-frequency one attributed to turbulence , and a high-frequency one ( 200-500 Hz ) attributed to bubble noise from water breaking the surface .
	manualset3
169899	8	413050	7	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The window lies between two noise sources , a low-frequency one attributed to turbulence , and a high-frequency one ( 200-500 Hz ) attributed to bubble noise from water breaking the surface .
	manualset3
169900	9	413050	7	NULL	NULL	0	NULL	surface	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The window lies between two noise sources , a low-frequency one attributed to turbulence , and a high-frequency one ( 200-500 Hz ) attributed to bubble noise from water breaking the surface .
	manualset3
169901	1	413051	7	NULL	NULL	0	NULL	within-run precision	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The within-run precision with buffer-based calibrators was below 8 % over the working range of PAPP-A ( 40-10000 mIU/l ) and beta-hCG ( 7.3-525 micrograms/l ) and no hook effect was observed .
	manualset3
169902	2	413051	7	NULL	NULL	0	NULL	buffer-based calibrators	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The within-run precision with buffer-based calibrators was below 8 % over the working range of PAPP-A ( 40-10000 mIU/l ) and beta-hCG ( 7.3-525 micrograms/l ) and no hook effect was observed .
	manualset3
169903	3	413051	7	NULL	NULL	0	NULL	 8 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The within-run precision with buffer-based calibrators was below 8 % over the working range of PAPP-A ( 40-10000 mIU/l ) and beta-hCG ( 7.3-525 micrograms/l ) and no hook effect was observed .
	manualset3
169904	4	413051	7	NULL	NULL	0	NULL	working range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The within-run precision with buffer-based calibrators was below 8 % over the working range of PAPP-A ( 40-10000 mIU/l ) and beta-hCG ( 7.3-525 micrograms/l ) and no hook effect was observed .
	manualset3
169905	5	413051	7	NULL	NULL	0	NULL	PAPP-A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The within-run precision with buffer-based calibrators was below 8 % over the working range of PAPP-A ( 40-10000 mIU/l ) and beta-hCG ( 7.3-525 micrograms/l ) and no hook effect was observed .
	manualset3
169906	6	413051	7	NULL	NULL	0	NULL	40-10000 mIU/l	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The within-run precision with buffer-based calibrators was below 8 % over the working range of PAPP-A ( 40-10000 mIU/l ) and beta-hCG ( 7.3-525 micrograms/l ) and no hook effect was observed .
	manualset3
169907	7	413051	7	NULL	NULL	0	NULL	beta-hCG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The within-run precision with buffer-based calibrators was below 8 % over the working range of PAPP-A ( 40-10000 mIU/l ) and beta-hCG ( 7.3-525 micrograms/l ) and no hook effect was observed .
	manualset3
169908	8	413051	7	NULL	NULL	0	NULL	7.3-525 micrograms/l	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The within-run precision with buffer-based calibrators was below 8 % over the working range of PAPP-A ( 40-10000 mIU/l ) and beta-hCG ( 7.3-525 micrograms/l ) and no hook effect was observed .
	manualset3
169909	9	413051	7	NULL	NULL	0	NULL	 hook effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The within-run precision with buffer-based calibrators was below 8 % over the working range of PAPP-A ( 40-10000 mIU/l ) and beta-hCG ( 7.3-525 micrograms/l ) and no hook effect was observed .
	manualset3
169910	1	413052	7	NULL	NULL	0	NULL	 work	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The work defines structure-activity relationships of C-terminal host defense peptides of thrombin and delineates a strategy for selecting peptide epitopes of therapeutic interest .
	manualset3
169911	2	413052	7	NULL	NULL	0	NULL	structure-activity relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The work defines structure-activity relationships of C-terminal host defense peptides of thrombin and delineates a strategy for selecting peptide epitopes of therapeutic interest .
	manualset3
169912	3	413052	7	NULL	NULL	0	NULL	C-terminal host defense peptides 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The work defines structure-activity relationships of C-terminal host defense peptides of thrombin and delineates a strategy for selecting peptide epitopes of therapeutic interest .
	manualset3
169913	4	413052	7	NULL	NULL	0	NULL	thrombin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The work defines structure-activity relationships of C-terminal host defense peptides of thrombin and delineates a strategy for selecting peptide epitopes of therapeutic interest .
	manualset3
169914	5	413052	7	NULL	NULL	0	NULL	strategy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The work defines structure-activity relationships of C-terminal host defense peptides of thrombin and delineates a strategy for selecting peptide epitopes of therapeutic interest .
	manualset3
169915	6	413052	7	NULL	NULL	0	NULL	peptide epitopes	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The work defines structure-activity relationships of C-terminal host defense peptides of thrombin and delineates a strategy for selecting peptide epitopes of therapeutic interest .
	manualset3
169916	7	413052	7	NULL	NULL	0	NULL	therapeutic interest	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The work defines structure-activity relationships of C-terminal host defense peptides of thrombin and delineates a strategy for selecting peptide epitopes of therapeutic interest .
	manualset3
169917	1	413053	7	NULL	NULL	0	NULL	work 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The work is useful for further research on the diagnosis of early breast cancers .
	manualset3
169918	2	413053	7	NULL	NULL	0	NULL	 research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The work is useful for further research on the diagnosis of early breast cancers .
	manualset3
169919	3	413053	7	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The work is useful for further research on the diagnosis of early breast cancers .
	manualset3
169920	4	413053	7	NULL	NULL	NULL	NULL	early breast cancers	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The work is useful for further research on the diagnosis of early breast cancers .
	manualset3
169921	1	413054	7	NULL	NULL	0	NULL	Activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of CD4 ( + ) T cells from GM3 synthase-null mice , deficient in GM3-derived gangliosides , is severely compromised , whereas CD8 ( + ) T-cell activation is normal .
	manualset3
169922	2	413054	7	NULL	NULL	0	NULL	CD4 ( + ) T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of CD4 ( + ) T cells from GM3 synthase-null mice , deficient in GM3-derived gangliosides , is severely compromised , whereas CD8 ( + ) T-cell activation is normal .
	manualset3
169923	3	413054	7	NULL	NULL	0	NULL	GM3 synthase-null mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of CD4 ( + ) T cells from GM3 synthase-null mice , deficient in GM3-derived gangliosides , is severely compromised , whereas CD8 ( + ) T-cell activation is normal .
	manualset3
169924	4	413054	7	NULL	NULL	0	NULL	GM3-derived gangliosides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of CD4 ( + ) T cells from GM3 synthase-null mice , deficient in GM3-derived gangliosides , is severely compromised , whereas CD8 ( + ) T-cell activation is normal .
	manualset3
169925	5	413054	7	NULL	NULL	0	NULL	CD8 ( + ) T-cell activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of CD4 ( + ) T cells from GM3 synthase-null mice , deficient in GM3-derived gangliosides , is severely compromised , whereas CD8 ( + ) T-cell activation is normal .
	manualset3
169926	1	413055	7	NULL	NULL	0	NULL	working environment	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The working environment is an important determinant of employee well-being .
	manualset3
169927	2	413055	7	NULL	NULL	0	NULL	determinant	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The working environment is an important determinant of employee well-being .
	manualset3
169928	3	413055	7	NULL	NULL	0	NULL	employee well-being	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The working environment is an important determinant of employee well-being .
	manualset3
169929	1	413056	7	NULL	NULL	0	NULL	 working hypothesis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The working hypothesis was that the homologous insect cells would utilize their inherent deoxyribonucleic acid ( DNA ) repair mechanism ( s ) to prevent , repair , or at least mitigate the damaging effects of UV-B light on viral DNA synthesis .
	manualset3
169930	2	413056	7	NULL	NULL	0	NULL	homologous insect cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The working hypothesis was that the homologous insect cells would utilize their inherent deoxyribonucleic acid ( DNA ) repair mechanism ( s ) to prevent , repair , or at least mitigate the damaging effects of UV-B light on viral DNA synthesis .
	manualset3
169931	3	413056	7	NULL	NULL	0	NULL	inherent deoxyribonucleic acid ( DNA ) repair mechanism ( s )	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The working hypothesis was that the homologous insect cells would utilize their inherent deoxyribonucleic acid ( DNA ) repair mechanism ( s ) to prevent , repair , or at least mitigate the damaging effects of UV-B light on viral DNA synthesis .
	manualset3
169935	7	413056	7	NULL	NULL	0	NULL	damaging effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The working hypothesis was that the homologous insect cells would utilize their inherent deoxyribonucleic acid ( DNA ) repair mechanism ( s ) to prevent , repair , or at least mitigate the damaging effects of UV-B light on viral DNA synthesis .
	manualset3
169936	8	413056	7	NULL	NULL	0	NULL	UV-B light	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The working hypothesis was that the homologous insect cells would utilize their inherent deoxyribonucleic acid ( DNA ) repair mechanism ( s ) to prevent , repair , or at least mitigate the damaging effects of UV-B light on viral DNA synthesis .
	manualset3
169937	9	413056	7	NULL	NULL	0	NULL	viral DNA synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The working hypothesis was that the homologous insect cells would utilize their inherent deoxyribonucleic acid ( DNA ) repair mechanism ( s ) to prevent , repair , or at least mitigate the damaging effects of UV-B light on viral DNA synthesis .
	manualset3
169938	1	413057	7	NULL	NULL	0	NULL	 wrinkle period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The wrinkle period has been reduced to about 600 nm on an ultrathin Au upper-layer/polystyrene ( PS ) underlay system .
	manualset3
169939	2	413057	7	NULL	NULL	0	NULL	600 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The wrinkle period has been reduced to about 600 nm on an ultrathin Au upper-layer/polystyrene ( PS ) underlay system .
	manualset3
169940	3	413057	7	NULL	NULL	0	NULL	ultrathin Au upper-layer/polystyrene ( PS ) underlay system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The wrinkle period has been reduced to about 600 nm on an ultrathin Au upper-layer/polystyrene ( PS ) underlay system .
	manualset3
169941	1	413058	7	NULL	NULL	0	NULL	 xeroderma pigmentosum group D ( XPD ) helicase subunit	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The xeroderma pigmentosum group D ( XPD ) helicase subunit of TFIIH functions in DNA repair and transcription initiation .
	manualset3
169942	2	413058	7	NULL	NULL	0	NULL	TFIIH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The xeroderma pigmentosum group D ( XPD ) helicase subunit of TFIIH functions in DNA repair and transcription initiation .
	manualset3
169943	3	413058	7	NULL	NULL	0	NULL	DNA repair	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The xeroderma pigmentosum group D ( XPD ) helicase subunit of TFIIH functions in DNA repair and transcription initiation .
	manualset3
169944	4	413058	7	NULL	NULL	0	NULL	transcription initiation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The xeroderma pigmentosum group D ( XPD ) helicase subunit of TFIIH functions in DNA repair and transcription initiation .
	manualset3
169945	1	413059	7	NULL	NULL	0	NULL	yeast CDC9 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The yeast CDC9 gene encodes both a nuclear and a mitochondrial form of DNA ligase I .
	manualset3
169946	2	413059	7	NULL	NULL	0	NULL	nuclear form	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The yeast CDC9 gene encodes both a nuclear and a mitochondrial form of DNA ligase I .
	manualset3
169947	3	413059	7	NULL	NULL	0	NULL	mitochondrial form	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The yeast CDC9 gene encodes both a nuclear and a mitochondrial form of DNA ligase I .
	manualset3
169948	4	413059	7	NULL	NULL	0	NULL	 DNA ligase I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The yeast CDC9 gene encodes both a nuclear and a mitochondrial form of DNA ligase I .
	manualset3
169949	1	413060	7	NULL	NULL	0	NULL	yeast Cbp1 protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The yeast Cbp1 protein , which is encoded by the nuclear CBP1 gene , is required for the stabilization of COB mRNA .
	manualset3
169950	2	413060	7	NULL	NULL	0	NULL	nuclear CBP1 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The yeast Cbp1 protein , which is encoded by the nuclear CBP1 gene , is required for the stabilization of COB mRNA .
	manualset3
169951	3	413060	7	NULL	NULL	0	NULL	stabilization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The yeast Cbp1 protein , which is encoded by the nuclear CBP1 gene , is required for the stabilization of COB mRNA .
	manualset3
169952	4	413060	7	NULL	NULL	0	NULL	COB mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The yeast Cbp1 protein , which is encoded by the nuclear CBP1 gene , is required for the stabilization of COB mRNA .
	manualset3
169953	1	413061	7	NULL	NULL	0	NULL	 yeast sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The yeast sequences are cleaved at only two sites , both of which map to regulatory regions : ( 1 ) the autonomously replicating sequence ( ARS ) , an origin of DNA replication , of the two micron plasmid and ( 2 ) the transcription terminator region of the LEU2 gene .
	manualset3
169954	2	413061	7	NULL	NULL	0	NULL	two sites	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The yeast sequences are cleaved at only two sites , both of which map to regulatory regions : ( 1 ) the autonomously replicating sequence ( ARS ) , an origin of DNA replication , of the two micron plasmid and ( 2 ) the transcription terminator region of the LEU2 gene .
	manualset3
169955	3	413061	7	NULL	NULL	0	NULL	regulatory regions	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The yeast sequences are cleaved at only two sites , both of which map to regulatory regions : ( 1 ) the autonomously replicating sequence ( ARS ) , an origin of DNA replication , of the two micron plasmid and ( 2 ) the transcription terminator region of the LEU2 gene .
	manualset3
169956	4	413061	7	NULL	NULL	0	NULL	autonomously replicating sequence ( ARS )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The yeast sequences are cleaved at only two sites , both of which map to regulatory regions : ( 1 ) the autonomously replicating sequence ( ARS ) , an origin of DNA replication , of the two micron plasmid and ( 2 ) the transcription terminator region of the LEU2 gene .
	manualset3
169957	5	413061	7	NULL	NULL	0	NULL	origin	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The yeast sequences are cleaved at only two sites , both of which map to regulatory regions : ( 1 ) the autonomously replicating sequence ( ARS ) , an origin of DNA replication , of the two micron plasmid and ( 2 ) the transcription terminator region of the LEU2 gene .
	manualset3
169958	6	413061	7	NULL	NULL	0	NULL	DNA replication	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The yeast sequences are cleaved at only two sites , both of which map to regulatory regions : ( 1 ) the autonomously replicating sequence ( ARS ) , an origin of DNA replication , of the two micron plasmid and ( 2 ) the transcription terminator region of the LEU2 gene .
	manualset3
169959	7	413061	7	NULL	NULL	0	NULL	 two micron plasmid	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The yeast sequences are cleaved at only two sites , both of which map to regulatory regions : ( 1 ) the autonomously replicating sequence ( ARS ) , an origin of DNA replication , of the two micron plasmid and ( 2 ) the transcription terminator region of the LEU2 gene .
	manualset3
169960	8	413061	7	NULL	NULL	0	NULL	 transcription terminator region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The yeast sequences are cleaved at only two sites , both of which map to regulatory regions : ( 1 ) the autonomously replicating sequence ( ARS ) , an origin of DNA replication , of the two micron plasmid and ( 2 ) the transcription terminator region of the LEU2 gene .
	manualset3
169961	9	413061	7	NULL	NULL	0	NULL	LEU2 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The yeast sequences are cleaved at only two sites , both of which map to regulatory regions : ( 1 ) the autonomously replicating sequence ( ARS ) , an origin of DNA replication , of the two micron plasmid and ( 2 ) the transcription terminator region of the LEU2 gene .
	manualset3
169962	1	413062	7	NULL	NULL	0	NULL	 yolk diameter	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The yolk diameter of cortisol-treated tilapia ( Oreochromis mossambicus ) larvae , immersed in freshwater ( FW ) containing 10 mg L-1 cortisol from 48 h postfertilization to 12 d posthatching , was significantly larger than that of control larvae after 8 d of treatment , suggesting that inhibition on larval growth occurred only after a long-term treatment with cortisol .
	manualset3
169963	2	413062	7	NULL	NULL	0	NULL	cortisol-treated tilapia ( Oreochromis mossambicus ) larvae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The yolk diameter of cortisol-treated tilapia ( Oreochromis mossambicus ) larvae , immersed in freshwater ( FW ) containing 10 mg L-1 cortisol from 48 h postfertilization to 12 d posthatching , was significantly larger than that of control larvae after 8 d of treatment , suggesting that inhibition on larval growth occurred only after a long-term treatment with cortisol .
	manualset3
169964	3	413062	7	NULL	NULL	0	NULL	freshwater ( FW )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The yolk diameter of cortisol-treated tilapia ( Oreochromis mossambicus ) larvae , immersed in freshwater ( FW ) containing 10 mg L-1 cortisol from 48 h postfertilization to 12 d posthatching , was significantly larger than that of control larvae after 8 d of treatment , suggesting that inhibition on larval growth occurred only after a long-term treatment with cortisol .
	manualset3
169965	4	413062	7	NULL	NULL	0	NULL	10 mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The yolk diameter of cortisol-treated tilapia ( Oreochromis mossambicus ) larvae , immersed in freshwater ( FW ) containing 10 mg L-1 cortisol from 48 h postfertilization to 12 d posthatching , was significantly larger than that of control larvae after 8 d of treatment , suggesting that inhibition on larval growth occurred only after a long-term treatment with cortisol .
	manualset3
169966	5	413062	7	NULL	NULL	0	NULL	L-1 cortisol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The yolk diameter of cortisol-treated tilapia ( Oreochromis mossambicus ) larvae , immersed in freshwater ( FW ) containing 10 mg L-1 cortisol from 48 h postfertilization to 12 d posthatching , was significantly larger than that of control larvae after 8 d of treatment , suggesting that inhibition on larval growth occurred only after a long-term treatment with cortisol .
	manualset3
169967	6	413062	7	NULL	NULL	0	NULL	48 h 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The yolk diameter of cortisol-treated tilapia ( Oreochromis mossambicus ) larvae , immersed in freshwater ( FW ) containing 10 mg L-1 cortisol from 48 h postfertilization to 12 d posthatching , was significantly larger than that of control larvae after 8 d of treatment , suggesting that inhibition on larval growth occurred only after a long-term treatment with cortisol .
	manualset3
169968	7	413062	7	NULL	NULL	0	NULL	postfertilization 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The yolk diameter of cortisol-treated tilapia ( Oreochromis mossambicus ) larvae , immersed in freshwater ( FW ) containing 10 mg L-1 cortisol from 48 h postfertilization to 12 d posthatching , was significantly larger than that of control larvae after 8 d of treatment , suggesting that inhibition on larval growth occurred only after a long-term treatment with cortisol .
	manualset3
169969	8	413062	7	NULL	NULL	0	NULL	12 d	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The yolk diameter of cortisol-treated tilapia ( Oreochromis mossambicus ) larvae , immersed in freshwater ( FW ) containing 10 mg L-1 cortisol from 48 h postfertilization to 12 d posthatching , was significantly larger than that of control larvae after 8 d of treatment , suggesting that inhibition on larval growth occurred only after a long-term treatment with cortisol .
	manualset3
169970	9	413062	7	NULL	NULL	0	NULL	posthatching 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The yolk diameter of cortisol-treated tilapia ( Oreochromis mossambicus ) larvae , immersed in freshwater ( FW ) containing 10 mg L-1 cortisol from 48 h postfertilization to 12 d posthatching , was significantly larger than that of control larvae after 8 d of treatment , suggesting that inhibition on larval growth occurred only after a long-term treatment with cortisol .
	manualset3
169971	10	413062	7	NULL	NULL	0	NULL	control larvae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The yolk diameter of cortisol-treated tilapia ( Oreochromis mossambicus ) larvae , immersed in freshwater ( FW ) containing 10 mg L-1 cortisol from 48 h postfertilization to 12 d posthatching , was significantly larger than that of control larvae after 8 d of treatment , suggesting that inhibition on larval growth occurred only after a long-term treatment with cortisol .
	manualset3
169972	11	413062	7	NULL	NULL	0	NULL	 8 d	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The yolk diameter of cortisol-treated tilapia ( Oreochromis mossambicus ) larvae , immersed in freshwater ( FW ) containing 10 mg L-1 cortisol from 48 h postfertilization to 12 d posthatching , was significantly larger than that of control larvae after 8 d of treatment , suggesting that inhibition on larval growth occurred only after a long-term treatment with cortisol .
	manualset3
169973	12	413062	7	NULL	NULL	NULL	NULL	treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The yolk diameter of cortisol-treated tilapia ( Oreochromis mossambicus ) larvae , immersed in freshwater ( FW ) containing 10 mg L-1 cortisol from 48 h postfertilization to 12 d posthatching , was significantly larger than that of control larvae after 8 d of treatment , suggesting that inhibition on larval growth occurred only after a long-term treatment with cortisol .
	manualset3
169974	13	413062	7	NULL	NULL	0	NULL	inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The yolk diameter of cortisol-treated tilapia ( Oreochromis mossambicus ) larvae , immersed in freshwater ( FW ) containing 10 mg L-1 cortisol from 48 h postfertilization to 12 d posthatching , was significantly larger than that of control larvae after 8 d of treatment , suggesting that inhibition on larval growth occurred only after a long-term treatment with cortisol .
	manualset3
169975	14	413062	7	NULL	NULL	0	NULL	larval growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The yolk diameter of cortisol-treated tilapia ( Oreochromis mossambicus ) larvae , immersed in freshwater ( FW ) containing 10 mg L-1 cortisol from 48 h postfertilization to 12 d posthatching , was significantly larger than that of control larvae after 8 d of treatment , suggesting that inhibition on larval growth occurred only after a long-term treatment with cortisol .
	manualset3
169976	15	413062	7	NULL	NULL	0	NULL	long-term treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The yolk diameter of cortisol-treated tilapia ( Oreochromis mossambicus ) larvae , immersed in freshwater ( FW ) containing 10 mg L-1 cortisol from 48 h postfertilization to 12 d posthatching , was significantly larger than that of control larvae after 8 d of treatment , suggesting that inhibition on larval growth occurred only after a long-term treatment with cortisol .
	manualset3
169977	16	413062	7	NULL	NULL	0	NULL	cortisol 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The yolk diameter of cortisol-treated tilapia ( Oreochromis mossambicus ) larvae , immersed in freshwater ( FW ) containing 10 mg L-1 cortisol from 48 h postfertilization to 12 d posthatching , was significantly larger than that of control larvae after 8 d of treatment , suggesting that inhibition on larval growth occurred only after a long-term treatment with cortisol .
	manualset3
169978	1	413063	7	NULL	NULL	0	NULL	Activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of CPP32-like caspases contributes to neuronal apoptosis and neurological dysfunction after traumatic brain injury .
	manualset3
169979	2	413063	7	NULL	NULL	0	NULL	CPP32-like caspases	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of CPP32-like caspases contributes to neuronal apoptosis and neurological dysfunction after traumatic brain injury .
	manualset3
169980	3	413063	7	NULL	NULL	0	NULL	neuronal apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of CPP32-like caspases contributes to neuronal apoptosis and neurological dysfunction after traumatic brain injury .
	manualset3
169981	4	413063	7	NULL	NULL	0	NULL	neurological dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of CPP32-like caspases contributes to neuronal apoptosis and neurological dysfunction after traumatic brain injury .
	manualset3
169982	5	413063	7	NULL	NULL	0	NULL	traumatic brain injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of CPP32-like caspases contributes to neuronal apoptosis and neurological dysfunction after traumatic brain injury .
	manualset3
169983	1	413064	7	NULL	NULL	0	NULL	 zip1 mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The zip1 mutation confers a uniform arrest in meiosis prior to the first division .
	manualset3
169984	2	413064	7	NULL	NULL	0	NULL	 uniform arrest	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The zip1 mutation confers a uniform arrest in meiosis prior to the first division .
	manualset3
169985	3	413064	7	NULL	NULL	0	NULL	meiosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The zip1 mutation confers a uniform arrest in meiosis prior to the first division .
	manualset3
169986	4	413064	7	NULL	NULL	0	NULL	first division	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The zip1 mutation confers a uniform arrest in meiosis prior to the first division .
	manualset3
169987	1	413065	7	NULL	NULL	0	NULL	neutrophils	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Their neutrophils are markedly deficient in secondary granules and vesicles and the empty cytoplasm appears gray on peripheral blood smears .
	manualset3
169988	2	413065	7	NULL	NULL	0	NULL	secondary granules	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Their neutrophils are markedly deficient in secondary granules and vesicles and the empty cytoplasm appears gray on peripheral blood smears .
	manualset3
169989	3	413065	7	NULL	NULL	0	NULL	 vesicles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Their neutrophils are markedly deficient in secondary granules and vesicles and the empty cytoplasm appears gray on peripheral blood smears .
	manualset3
169990	4	413065	7	NULL	NULL	0	NULL	empty cytoplasm	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Their neutrophils are markedly deficient in secondary granules and vesicles and the empty cytoplasm appears gray on peripheral blood smears .
	manualset3
169991	5	413065	7	NULL	NULL	0	NULL	gray	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Their neutrophils are markedly deficient in secondary granules and vesicles and the empty cytoplasm appears gray on peripheral blood smears .
	manualset3
169992	6	413065	7	NULL	NULL	0	NULL	peripheral blood smears	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Their neutrophils are markedly deficient in secondary granules and vesicles and the empty cytoplasm appears gray on peripheral blood smears .
	manualset3
169993	1	413066	7	NULL	NULL	0	NULL	performance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Their performance was evaluated by the number of steps and the running time in the last step .
	manualset3
169994	2	413066	7	NULL	NULL	0	NULL	 number of steps	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Their performance was evaluated by the number of steps and the running time in the last step .
	manualset3
169995	3	413066	7	NULL	NULL	0	NULL	running time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Their performance was evaluated by the number of steps and the running time in the last step .
	manualset3
169996	4	413066	7	NULL	NULL	0	NULL	last step	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Their performance was evaluated by the number of steps and the running time in the last step .
	manualset3
169997	1	413067	7	NULL	NULL	0	NULL	 pregnancies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Their pregnancies are considered to be of low risk compared with pregnancies in women with systemic inflammatory connective tissue disease .
	manualset3
169998	2	413067	7	NULL	NULL	0	NULL	low risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Their pregnancies are considered to be of low risk compared with pregnancies in women with systemic inflammatory connective tissue disease .
	manualset3
169999	3	413067	7	NULL	NULL	0	NULL	pregnancies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Their pregnancies are considered to be of low risk compared with pregnancies in women with systemic inflammatory connective tissue disease .
	manualset3
170000	4	413067	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Their pregnancies are considered to be of low risk compared with pregnancies in women with systemic inflammatory connective tissue disease .
	manualset3
170001	5	413067	7	NULL	NULL	0	NULL	systemic inflammatory connective tissue disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Their pregnancies are considered to be of low risk compared with pregnancies in women with systemic inflammatory connective tissue disease .
	manualset3
170002	1	413068	7	NULL	NULL	0	NULL	structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Their structures were established as isotrilobine ( I ) , trilobine ( II ) , isotrilobine-N-2-oxide ( III ) and nortrilobine ( IV ) on the basis of spectral analysis ( UV , IR , HNMR , MS ) , physico-chemical constants and properties of the derivatives .
	manualset3
170003	2	413068	7	NULL	NULL	0	NULL	 isotrilobine ( I )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Their structures were established as isotrilobine ( I ) , trilobine ( II ) , isotrilobine-N-2-oxide ( III ) and nortrilobine ( IV ) on the basis of spectral analysis ( UV , IR , HNMR , MS ) , physico-chemical constants and properties of the derivatives .
	manualset3
170004	3	413068	7	NULL	NULL	0	NULL	trilobine ( II )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Their structures were established as isotrilobine ( I ) , trilobine ( II ) , isotrilobine-N-2-oxide ( III ) and nortrilobine ( IV ) on the basis of spectral analysis ( UV , IR , HNMR , MS ) , physico-chemical constants and properties of the derivatives .
	manualset3
170005	4	413068	7	NULL	NULL	0	NULL	isotrilobine-N-2-oxide ( III )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Their structures were established as isotrilobine ( I ) , trilobine ( II ) , isotrilobine-N-2-oxide ( III ) and nortrilobine ( IV ) on the basis of spectral analysis ( UV , IR , HNMR , MS ) , physico-chemical constants and properties of the derivatives .
	manualset3
170006	5	413068	7	NULL	NULL	0	NULL	nortrilobine ( IV )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Their structures were established as isotrilobine ( I ) , trilobine ( II ) , isotrilobine-N-2-oxide ( III ) and nortrilobine ( IV ) on the basis of spectral analysis ( UV , IR , HNMR , MS ) , physico-chemical constants and properties of the derivatives .
	manualset3
170007	6	413068	7	NULL	NULL	0	NULL	basis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Their structures were established as isotrilobine ( I ) , trilobine ( II ) , isotrilobine-N-2-oxide ( III ) and nortrilobine ( IV ) on the basis of spectral analysis ( UV , IR , HNMR , MS ) , physico-chemical constants and properties of the derivatives .
	manualset3
170008	7	413068	7	NULL	NULL	0	NULL	spectral analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Their structures were established as isotrilobine ( I ) , trilobine ( II ) , isotrilobine-N-2-oxide ( III ) and nortrilobine ( IV ) on the basis of spectral analysis ( UV , IR , HNMR , MS ) , physico-chemical constants and properties of the derivatives .
	manualset3
170009	8	413068	7	NULL	NULL	0	NULL	UV , IR , HNMR , MS	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Their structures were established as isotrilobine ( I ) , trilobine ( II ) , isotrilobine-N-2-oxide ( III ) and nortrilobine ( IV ) on the basis of spectral analysis ( UV , IR , HNMR , MS ) , physico-chemical constants and properties of the derivatives .
	manualset3
170010	9	413068	7	NULL	NULL	0	NULL	physico-chemical constants	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Their structures were established as isotrilobine ( I ) , trilobine ( II ) , isotrilobine-N-2-oxide ( III ) and nortrilobine ( IV ) on the basis of spectral analysis ( UV , IR , HNMR , MS ) , physico-chemical constants and properties of the derivatives .
	manualset3
170011	10	413068	7	NULL	NULL	0	NULL	properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Their structures were established as isotrilobine ( I ) , trilobine ( II ) , isotrilobine-N-2-oxide ( III ) and nortrilobine ( IV ) on the basis of spectral analysis ( UV , IR , HNMR , MS ) , physico-chemical constants and properties of the derivatives .
	manualset3
170012	11	413068	7	NULL	NULL	0	NULL	derivatives	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Their structures were established as isotrilobine ( I ) , trilobine ( II ) , isotrilobine-N-2-oxide ( III ) and nortrilobine ( IV ) on the basis of spectral analysis ( UV , IR , HNMR , MS ) , physico-chemical constants and properties of the derivatives .
	manualset3
170013	1	413069	7	NULL	NULL	0	NULL	Activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of G proteins by treatment with aluminum fluoride produced an accumulation within the erythrocyte cytosol of vesicles coated with Plasmodium homologs of COPII and N-ethylmaleimide-sensitive factor , proteins involved in intracellular transport between the Golgi apparatus and the endoplasmic reticulum .
	manualset3
170014	2	413069	7	NULL	NULL	0	NULL	G proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of G proteins by treatment with aluminum fluoride produced an accumulation within the erythrocyte cytosol of vesicles coated with Plasmodium homologs of COPII and N-ethylmaleimide-sensitive factor , proteins involved in intracellular transport between the Golgi apparatus and the endoplasmic reticulum .
	manualset3
170015	3	413069	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of G proteins by treatment with aluminum fluoride produced an accumulation within the erythrocyte cytosol of vesicles coated with Plasmodium homologs of COPII and N-ethylmaleimide-sensitive factor , proteins involved in intracellular transport between the Golgi apparatus and the endoplasmic reticulum .
	manualset3
170016	4	413069	7	NULL	NULL	0	NULL	aluminum fluoride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of G proteins by treatment with aluminum fluoride produced an accumulation within the erythrocyte cytosol of vesicles coated with Plasmodium homologs of COPII and N-ethylmaleimide-sensitive factor , proteins involved in intracellular transport between the Golgi apparatus and the endoplasmic reticulum .
	manualset3
170017	5	413069	7	NULL	NULL	0	NULL	accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of G proteins by treatment with aluminum fluoride produced an accumulation within the erythrocyte cytosol of vesicles coated with Plasmodium homologs of COPII and N-ethylmaleimide-sensitive factor , proteins involved in intracellular transport between the Golgi apparatus and the endoplasmic reticulum .
	manualset3
170018	6	413069	7	NULL	NULL	0	NULL	erythrocyte cytosol 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of G proteins by treatment with aluminum fluoride produced an accumulation within the erythrocyte cytosol of vesicles coated with Plasmodium homologs of COPII and N-ethylmaleimide-sensitive factor , proteins involved in intracellular transport between the Golgi apparatus and the endoplasmic reticulum .
	manualset3
170019	7	413069	7	NULL	NULL	0	NULL	 vesicles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of G proteins by treatment with aluminum fluoride produced an accumulation within the erythrocyte cytosol of vesicles coated with Plasmodium homologs of COPII and N-ethylmaleimide-sensitive factor , proteins involved in intracellular transport between the Golgi apparatus and the endoplasmic reticulum .
	manualset3
170020	8	413069	7	NULL	NULL	0	NULL	Plasmodium homologs of COPII	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of G proteins by treatment with aluminum fluoride produced an accumulation within the erythrocyte cytosol of vesicles coated with Plasmodium homologs of COPII and N-ethylmaleimide-sensitive factor , proteins involved in intracellular transport between the Golgi apparatus and the endoplasmic reticulum .
	manualset3
170021	9	413069	7	NULL	NULL	0	NULL	N-ethylmaleimide-sensitive factor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of G proteins by treatment with aluminum fluoride produced an accumulation within the erythrocyte cytosol of vesicles coated with Plasmodium homologs of COPII and N-ethylmaleimide-sensitive factor , proteins involved in intracellular transport between the Golgi apparatus and the endoplasmic reticulum .
	manualset3
170022	10	413069	7	NULL	NULL	0	NULL	proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of G proteins by treatment with aluminum fluoride produced an accumulation within the erythrocyte cytosol of vesicles coated with Plasmodium homologs of COPII and N-ethylmaleimide-sensitive factor , proteins involved in intracellular transport between the Golgi apparatus and the endoplasmic reticulum .
	manualset3
170023	11	413069	7	NULL	NULL	0	NULL	intracellular transport	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of G proteins by treatment with aluminum fluoride produced an accumulation within the erythrocyte cytosol of vesicles coated with Plasmodium homologs of COPII and N-ethylmaleimide-sensitive factor , proteins involved in intracellular transport between the Golgi apparatus and the endoplasmic reticulum .
	manualset3
170024	12	413069	7	NULL	NULL	0	NULL	 Golgi apparatus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of G proteins by treatment with aluminum fluoride produced an accumulation within the erythrocyte cytosol of vesicles coated with Plasmodium homologs of COPII and N-ethylmaleimide-sensitive factor , proteins involved in intracellular transport between the Golgi apparatus and the endoplasmic reticulum .
	manualset3
170025	13	413069	7	NULL	NULL	0	NULL	endoplasmic reticulum	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of G proteins by treatment with aluminum fluoride produced an accumulation within the erythrocyte cytosol of vesicles coated with Plasmodium homologs of COPII and N-ethylmaleimide-sensitive factor , proteins involved in intracellular transport between the Golgi apparatus and the endoplasmic reticulum .
	manualset3
170026	1	413070	7	NULL	NULL	0	NULL	XbaI 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Their XbaI , BlnI , and combined XbaI-BlnI PFGE patterns revealed levels of genetic similarity of 93 , 75 , and 90 % , respectively .
	manualset3
170027	2	413070	7	NULL	NULL	0	NULL	BlnI	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Their XbaI , BlnI , and combined XbaI-BlnI PFGE patterns revealed levels of genetic similarity of 93 , 75 , and 90 % , respectively .
	manualset3
170028	3	413070	7	NULL	NULL	0	NULL	XbaI-BlnI PFGE patterns	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Their XbaI , BlnI , and combined XbaI-BlnI PFGE patterns revealed levels of genetic similarity of 93 , 75 , and 90 % , respectively .
	manualset3
170029	4	413070	7	NULL	NULL	0	NULL	 levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Their XbaI , BlnI , and combined XbaI-BlnI PFGE patterns revealed levels of genetic similarity of 93 , 75 , and 90 % , respectively .
	manualset3
170030	5	413070	7	NULL	NULL	0	NULL	genetic similarity	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Their XbaI , BlnI , and combined XbaI-BlnI PFGE patterns revealed levels of genetic similarity of 93 , 75 , and 90 % , respectively .
	manualset3
170031	6	413070	7	NULL	NULL	0	NULL	 93%	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Their XbaI , BlnI , and combined XbaI-BlnI PFGE patterns revealed levels of genetic similarity of 93 , 75 , and 90 % , respectively .
	manualset3
170032	7	413070	7	NULL	NULL	0	NULL	75%	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Their XbaI , BlnI , and combined XbaI-BlnI PFGE patterns revealed levels of genetic similarity of 93 , 75 , and 90 % , respectively .
	manualset3
170033	8	413070	7	NULL	NULL	0	NULL	 90 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Their XbaI , BlnI , and combined XbaI-BlnI PFGE patterns revealed levels of genetic similarity of 93 , 75 , and 90 % , respectively .
	manualset3
170034	1	413071	7	NULL	NULL	0	NULL	 bindin	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Their bindin , however , is distinct and coalesces within each morphospecies .
	manualset3
170035	2	413071	7	NULL	NULL	0	NULL	morphospecies	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Their bindin , however , is distinct and coalesces within each morphospecies .
	manualset3
170036	1	413072	7	NULL	NULL	0	NULL	 binding sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Their binding sites were mapped to BH3 ( Bcl-2 homology ) domain of Puma and BH1 domain of Mcl-1 , respectively .
	manualset3
170037	2	413072	7	NULL	NULL	0	NULL	BH3 ( Bcl-2 homology ) domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Their binding sites were mapped to BH3 ( Bcl-2 homology ) domain of Puma and BH1 domain of Mcl-1 , respectively .
	manualset3
170038	3	413072	7	NULL	NULL	0	NULL	Puma	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Their binding sites were mapped to BH3 ( Bcl-2 homology ) domain of Puma and BH1 domain of Mcl-1 , respectively .
	manualset3
170039	4	413072	7	NULL	NULL	0	NULL	BH1 domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Their binding sites were mapped to BH3 ( Bcl-2 homology ) domain of Puma and BH1 domain of Mcl-1 , respectively .
	manualset3
170040	5	413072	7	NULL	NULL	0	NULL	Mcl-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Their binding sites were mapped to BH3 ( Bcl-2 homology ) domain of Puma and BH1 domain of Mcl-1 , respectively .
	manualset3
170041	1	413073	7	NULL	NULL	0	NULL	biodistribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Their biodistribution and intrahepatic distribution were subsequently investigated .
	manualset3
170042	2	413073	7	NULL	NULL	0	NULL	intrahepatic distribution 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Their biodistribution and intrahepatic distribution were subsequently investigated .
	manualset3
170043	1	413074	7	NULL	NULL	NULL	NULL	characteristic feature 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Their characteristic feature is the presence of extremely long and thin prolongations ( called telopodes ) .
	manualset3
170044	2	413074	7	NULL	NULL	NULL	NULL	presence	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Their characteristic feature is the presence of extremely long and thin prolongations ( called telopodes ) .
	manualset3
170045	3	413074	7	NULL	NULL	0	NULL	long and thin prolongations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Their characteristic feature is the presence of extremely long and thin prolongations ( called telopodes ) .
	manualset3
170046	4	413074	7	NULL	NULL	0	NULL	telopodes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Their characteristic feature is the presence of extremely long and thin prolongations ( called telopodes ) .
	manualset3
170047	1	413075	7	NULL	NULL	0	NULL	Comments	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comments on heart failure : resource utilization was accounted for ) .
	manualset3
170048	2	413075	7	NULL	NULL	0	NULL	heart failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comments on heart failure : resource utilization was accounted for ) .
	manualset3
170049	3	413075	7	NULL	NULL	0	NULL	resource utilization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comments on heart failure : resource utilization was accounted for ) .
	manualset3
170050	1	413076	7	NULL	NULL	0	NULL	Activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of Notch receptors by Jag-1 caused CBF1-dependent up-regulation of miR-143 / 145 , increased differentiation , and decreased proliferation .
	manualset3
170051	2	413076	7	NULL	NULL	NULL	NULL	Notch receptors	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Activation of Notch receptors by Jag-1 caused CBF1-dependent up-regulation of miR-143 / 145 , increased differentiation , and decreased proliferation .
	manualset3
170052	3	413076	7	NULL	NULL	0	NULL	Jag-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of Notch receptors by Jag-1 caused CBF1-dependent up-regulation of miR-143 / 145 , increased differentiation , and decreased proliferation .
	manualset3
170053	4	413076	7	NULL	NULL	0	NULL	CBF1-dependent up-regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of Notch receptors by Jag-1 caused CBF1-dependent up-regulation of miR-143 / 145 , increased differentiation , and decreased proliferation .
	manualset3
170054	5	413076	7	NULL	NULL	0	NULL	miR-143 / 145 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of Notch receptors by Jag-1 caused CBF1-dependent up-regulation of miR-143 / 145 , increased differentiation , and decreased proliferation .
	manualset3
170055	6	413076	7	NULL	NULL	NULL	NULL	increased differentiation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Activation of Notch receptors by Jag-1 caused CBF1-dependent up-regulation of miR-143 / 145 , increased differentiation , and decreased proliferation .
	manualset3
170056	7	413076	7	NULL	NULL	NULL	NULL	 decreased proliferation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Activation of Notch receptors by Jag-1 caused CBF1-dependent up-regulation of miR-143 / 145 , increased differentiation , and decreased proliferation .
	manualset3
170057	1	413077	7	NULL	NULL	0	NULL	binding protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Their common binding protein , GH binding protein ( GHBP ) , displays peak serum levels at mid-gestation in normal individuals .
	manualset3
170058	2	413077	7	NULL	NULL	0	NULL	GH binding protein ( GHBP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Their common binding protein , GH binding protein ( GHBP ) , displays peak serum levels at mid-gestation in normal individuals .
	manualset3
170059	3	413077	7	NULL	NULL	0	NULL	serum levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Their common binding protein , GH binding protein ( GHBP ) , displays peak serum levels at mid-gestation in normal individuals .
	manualset3
170060	4	413077	7	NULL	NULL	0	NULL	mid-gestation	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Their common binding protein , GH binding protein ( GHBP ) , displays peak serum levels at mid-gestation in normal individuals .
	manualset3
170061	5	413077	7	NULL	NULL	0	NULL	normal individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Their common binding protein , GH binding protein ( GHBP ) , displays peak serum levels at mid-gestation in normal individuals .
	manualset3
170062	1	413078	7	NULL	NULL	0	NULL	E ( 3 ) formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Their effect on E ( 3 ) formation was more pronounced than that on E ( 2 ) due to the lower affinity of 16-OHT than testosterone to aromatase .
	manualset3
170063	2	413078	7	NULL	NULL	0	NULL	E ( 2 )	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Their effect on E ( 3 ) formation was more pronounced than that on E ( 2 ) due to the lower affinity of 16-OHT than testosterone to aromatase .
	manualset3
170064	4	413078	7	NULL	NULL	NULL	NULL	16-OHT	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Their effect on E ( 3 ) formation was more pronounced than that on E ( 2 ) due to the lower affinity of 16-OHT than testosterone to aromatase .
	manualset3
170065	3	413078	7	NULL	NULL	0	NULL	lower affinity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Their effect on E ( 3 ) formation was more pronounced than that on E ( 2 ) due to the lower affinity of 16-OHT than testosterone to aromatase .
	manualset3
170066	5	413078	7	NULL	NULL	0	NULL	testosterone 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Their effect on E ( 3 ) formation was more pronounced than that on E ( 2 ) due to the lower affinity of 16-OHT than testosterone to aromatase .
	manualset3
170067	6	413078	7	NULL	NULL	0	NULL	aromatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Their effect on E ( 3 ) formation was more pronounced than that on E ( 2 ) due to the lower affinity of 16-OHT than testosterone to aromatase .
	manualset3
170068	1	413079	7	NULL	NULL	0	NULL	 inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Their inhibition results in cholinergic syndrome and death .
	manualset3
170069	2	413079	7	NULL	NULL	0	NULL	cholinergic syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Their inhibition results in cholinergic syndrome and death .
	manualset3
170070	3	413079	7	NULL	NULL	0	NULL	 death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Their inhibition results in cholinergic syndrome and death .
	manualset3
170071	1	413080	7	NULL	NULL	0	NULL	 needs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Their needs in relation to Dating and Intimacy were also significantly higher but no differences were found between groups in relation to sexual experience .
	manualset3
170072	2	413080	7	NULL	NULL	0	NULL	 relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Their needs in relation to Dating and Intimacy were also significantly higher but no differences were found between groups in relation to sexual experience .
	manualset3
170073	3	413080	7	NULL	NULL	0	NULL	Dating	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Their needs in relation to Dating and Intimacy were also significantly higher but no differences were found between groups in relation to sexual experience .
	manualset3
170074	4	413080	7	NULL	NULL	0	NULL	 Intimacy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Their needs in relation to Dating and Intimacy were also significantly higher but no differences were found between groups in relation to sexual experience .
	manualset3
170075	5	413080	7	NULL	NULL	0	NULL	 differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Their needs in relation to Dating and Intimacy were also significantly higher but no differences were found between groups in relation to sexual experience .
	manualset3
170076	6	413080	7	NULL	NULL	0	NULL	groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Their needs in relation to Dating and Intimacy were also significantly higher but no differences were found between groups in relation to sexual experience .
	manualset3
170077	7	413080	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Their needs in relation to Dating and Intimacy were also significantly higher but no differences were found between groups in relation to sexual experience .
	manualset3
170078	8	413080	7	NULL	NULL	0	NULL	 sexual experience	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Their needs in relation to Dating and Intimacy were also significantly higher but no differences were found between groups in relation to sexual experience .
	manualset3
170079	1	413081	7	NULL	NULL	0	NULL	 number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Their number and affinity to the radioligand ( 125I ) - cyanopindolol .
	manualset3
170080	2	413081	7	NULL	NULL	0	NULL	affinity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Their number and affinity to the radioligand ( 125I ) - cyanopindolol .
	manualset3
170081	3	413081	7	NULL	NULL	0	NULL	radioligand ( 125I ) - cyanopindolol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Their number and affinity to the radioligand ( 125I ) - cyanopindolol .
	manualset3
170082	1	413082	7	NULL	NULL	0	NULL	percentage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Their percentage within the total Treg pool strongly decreased after transplantation and remained relatively low during the first year after transplantation in all patients .
	manualset3
170083	2	413082	7	NULL	NULL	0	NULL	total Treg pool	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Their percentage within the total Treg pool strongly decreased after transplantation and remained relatively low during the first year after transplantation in all patients .
	manualset3
170084	3	413082	7	NULL	NULL	0	NULL	 transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Their percentage within the total Treg pool strongly decreased after transplantation and remained relatively low during the first year after transplantation in all patients .
	manualset3
170085	4	413082	7	NULL	NULL	0	NULL	first year	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Their percentage within the total Treg pool strongly decreased after transplantation and remained relatively low during the first year after transplantation in all patients .
	manualset3
170086	5	413082	7	NULL	NULL	0	NULL	transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Their percentage within the total Treg pool strongly decreased after transplantation and remained relatively low during the first year after transplantation in all patients .
	manualset3
170087	6	413082	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Their percentage within the total Treg pool strongly decreased after transplantation and remained relatively low during the first year after transplantation in all patients .
	manualset3
170088	1	413083	7	NULL	NULL	0	NULL	perfusion ventilation lung scintigraphy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Their perfusion ventilation lung scintigraphy demonstrated multiple defects , and gallium scintigraphy showed abnormal accumulation in both lungs , and the spleen .
	manualset3
170089	2	413083	7	NULL	NULL	0	NULL	multiple defects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Their perfusion ventilation lung scintigraphy demonstrated multiple defects , and gallium scintigraphy showed abnormal accumulation in both lungs , and the spleen .
	manualset3
170090	3	413083	7	NULL	NULL	0	NULL	gallium scintigraphy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Their perfusion ventilation lung scintigraphy demonstrated multiple defects , and gallium scintigraphy showed abnormal accumulation in both lungs , and the spleen .
	manualset3
170091	4	413083	7	NULL	NULL	0	NULL	abnormal accumulation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Their perfusion ventilation lung scintigraphy demonstrated multiple defects , and gallium scintigraphy showed abnormal accumulation in both lungs , and the spleen .
	manualset3
170092	5	413083	7	NULL	NULL	0	NULL	lungs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Their perfusion ventilation lung scintigraphy demonstrated multiple defects , and gallium scintigraphy showed abnormal accumulation in both lungs , and the spleen .
	manualset3
170093	6	413083	7	NULL	NULL	0	NULL	spleen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Their perfusion ventilation lung scintigraphy demonstrated multiple defects , and gallium scintigraphy showed abnormal accumulation in both lungs , and the spleen .
	manualset3
170094	1	413084	7	NULL	NULL	0	NULL	Activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of TCF/LEF signalling decreases factor withdrawal-induced apoptosis of normal progenitors .
	manualset3
170095	2	413084	7	NULL	NULL	0	NULL	TCF/LEF signalling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of TCF/LEF signalling decreases factor withdrawal-induced apoptosis of normal progenitors .
	manualset3
170096	3	413084	7	NULL	NULL	0	NULL	factor withdrawal-induced apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of TCF/LEF signalling decreases factor withdrawal-induced apoptosis of normal progenitors .
	manualset3
170097	4	413084	7	NULL	NULL	0	NULL	normal progenitors	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of TCF/LEF signalling decreases factor withdrawal-induced apoptosis of normal progenitors .
	manualset3
170098	1	413085	7	NULL	NULL	0	NULL	preparation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Their preparation , satisfaction , and outlook .
	manualset3
170099	2	413085	7	NULL	NULL	0	NULL	satisfaction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Their preparation , satisfaction , and outlook .
	manualset3
170100	3	413085	7	NULL	NULL	0	NULL	outlook	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Their preparation , satisfaction , and outlook .
	manualset3
170101	1	413086	7	NULL	NULL	0	NULL	putative protein products	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Their putative protein products have 47.6 and 45.5 % identities with hCKLFSF2 , respectively ; both of them contain four potential transmembrane regions and MARVEL domains , which are also similar with hCKLFSF2 .
	manualset3
170102	2	413086	7	NULL	NULL	0	NULL	 47.6% 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Their putative protein products have 47.6 and 45.5 % identities with hCKLFSF2 , respectively ; both of them contain four potential transmembrane regions and MARVEL domains , which are also similar with hCKLFSF2 .
	manualset3
170103	3	413086	7	NULL	NULL	0	NULL	45.5 % identities	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Their putative protein products have 47.6 and 45.5 % identities with hCKLFSF2 , respectively ; both of them contain four potential transmembrane regions and MARVEL domains , which are also similar with hCKLFSF2 .
	manualset3
170104	4	413086	7	NULL	NULL	0	NULL	hCKLFSF2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Their putative protein products have 47.6 and 45.5 % identities with hCKLFSF2 , respectively ; both of them contain four potential transmembrane regions and MARVEL domains , which are also similar with hCKLFSF2 .
	manualset3
170105	5	413086	7	NULL	NULL	0	NULL	four potential transmembrane regions	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Their putative protein products have 47.6 and 45.5 % identities with hCKLFSF2 , respectively ; both of them contain four potential transmembrane regions and MARVEL domains , which are also similar with hCKLFSF2 .
	manualset3
170106	6	413086	7	NULL	NULL	0	NULL	MARVEL domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Their putative protein products have 47.6 and 45.5 % identities with hCKLFSF2 , respectively ; both of them contain four potential transmembrane regions and MARVEL domains , which are also similar with hCKLFSF2 .
	manualset3
170108	8	413086	7	NULL	NULL	0	NULL	 hCKLFSF2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Their putative protein products have 47.6 and 45.5 % identities with hCKLFSF2 , respectively ; both of them contain four potential transmembrane regions and MARVEL domains , which are also similar with hCKLFSF2 .
	manualset3
170109	1	413087	7	NULL	NULL	0	NULL	 release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Their release by tumor cells may represent the future for targeting therapeutic interventions and for development of multiplexed diagnostic biomarkers .
	manualset3
170110	2	413087	7	NULL	NULL	0	NULL	tumor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Their release by tumor cells may represent the future for targeting therapeutic interventions and for development of multiplexed diagnostic biomarkers .
	manualset3
170111	3	413087	7	NULL	NULL	0	NULL	future	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Their release by tumor cells may represent the future for targeting therapeutic interventions and for development of multiplexed diagnostic biomarkers .
	manualset3
170112	4	413087	7	NULL	NULL	0	NULL	therapeutic interventions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Their release by tumor cells may represent the future for targeting therapeutic interventions and for development of multiplexed diagnostic biomarkers .
	manualset3
170113	5	413087	7	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Their release by tumor cells may represent the future for targeting therapeutic interventions and for development of multiplexed diagnostic biomarkers .
	manualset3
170114	6	413087	7	NULL	NULL	0	NULL	multiplexed diagnostic biomarkers	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Their release by tumor cells may represent the future for targeting therapeutic interventions and for development of multiplexed diagnostic biomarkers .
	manualset3
170115	1	413088	7	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Their role has been established in the diagnosis of injury , prognosis and the assessment of progress following repair .
	manualset3
170116	2	413088	7	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Their role has been established in the diagnosis of injury , prognosis and the assessment of progress following repair .
	manualset3
170117	3	413088	7	NULL	NULL	0	NULL	injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Their role has been established in the diagnosis of injury , prognosis and the assessment of progress following repair .
	manualset3
170118	4	413088	7	NULL	NULL	0	NULL	prognosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Their role has been established in the diagnosis of injury , prognosis and the assessment of progress following repair .
	manualset3
170119	5	413088	7	NULL	NULL	0	NULL	assessment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Their role has been established in the diagnosis of injury , prognosis and the assessment of progress following repair .
	manualset3
170120	6	413088	7	NULL	NULL	NULL	NULL	 progress	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Their role has been established in the diagnosis of injury , prognosis and the assessment of progress following repair .
	manualset3
170121	7	413088	7	NULL	NULL	NULL	NULL	 repair	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Their role has been established in the diagnosis of injury , prognosis and the assessment of progress following repair .
	manualset3
170122	1	413089	7	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Their role is to disorganize the mitotic spindle by targeting its main constituent , the microtubules , themselves made of heterodimers of alpha and beta-tubulin .
	manualset3
170123	2	413089	7	NULL	NULL	NULL	NULL	mitotic spindle	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Their role is to disorganize the mitotic spindle by targeting its main constituent , the microtubules , themselves made of heterodimers of alpha and beta-tubulin .
	manualset3
170124	3	413089	7	NULL	NULL	0	NULL	main constituent	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Their role is to disorganize the mitotic spindle by targeting its main constituent , the microtubules , themselves made of heterodimers of alpha and beta-tubulin .
	manualset3
170125	4	413089	7	NULL	NULL	0	NULL	 microtubules	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Their role is to disorganize the mitotic spindle by targeting its main constituent , the microtubules , themselves made of heterodimers of alpha and beta-tubulin .
	manualset3
170126	5	413089	7	NULL	NULL	0	NULL	heterodimers	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Their role is to disorganize the mitotic spindle by targeting its main constituent , the microtubules , themselves made of heterodimers of alpha and beta-tubulin .
	manualset3
170127	6	413089	7	NULL	NULL	0	NULL	alpha-tubulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Their role is to disorganize the mitotic spindle by targeting its main constituent , the microtubules , themselves made of heterodimers of alpha and beta-tubulin .
	manualset3
170128	7	413089	7	NULL	NULL	0	NULL	beta-tubulin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Their role is to disorganize the mitotic spindle by targeting its main constituent , the microtubules , themselves made of heterodimers of alpha and beta-tubulin .
	manualset3
170129	1	413090	7	NULL	NULL	0	NULL	serum IgG1 concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Their serum IgG1 concentrations before and after colostrum intake , were compared with IgG1 concentrations in conventionally reared lambs .
	manualset3
170132	4	413090	7	NULL	NULL	0	NULL	colostrum intake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Their serum IgG1 concentrations before and after colostrum intake , were compared with IgG1 concentrations in conventionally reared lambs .
	manualset3
170133	5	413090	7	NULL	NULL	0	NULL	IgG1 concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Their serum IgG1 concentrations before and after colostrum intake , were compared with IgG1 concentrations in conventionally reared lambs .
	manualset3
170134	6	413090	7	NULL	NULL	0	NULL	 reared lambs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Their serum IgG1 concentrations before and after colostrum intake , were compared with IgG1 concentrations in conventionally reared lambs .
	manualset3
170135	1	413091	7	NULL	NULL	0	NULL	size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Their size or localization in the tumor mass does not alter the good prognosis of this type of renal tumor .
	manualset3
170136	2	413091	7	NULL	NULL	0	NULL	 localization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Their size or localization in the tumor mass does not alter the good prognosis of this type of renal tumor .
	manualset3
170137	3	413091	7	NULL	NULL	0	NULL	tumor mass	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Their size or localization in the tumor mass does not alter the good prognosis of this type of renal tumor .
	manualset3
170138	4	413091	7	NULL	NULL	0	NULL	good prognosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Their size or localization in the tumor mass does not alter the good prognosis of this type of renal tumor .
	manualset3
170139	5	413091	7	NULL	NULL	0	NULL	 type	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Their size or localization in the tumor mass does not alter the good prognosis of this type of renal tumor .
	manualset3
170140	6	413091	7	NULL	NULL	0	NULL	renal tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Their size or localization in the tumor mass does not alter the good prognosis of this type of renal tumor .
	manualset3
170141	1	413092	7	NULL	NULL	0	NULL	specificity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Their specificity for RNA splicing instead of DNA is given by cytoplasmic proteins .
	manualset3
170142	2	413092	7	NULL	NULL	0	NULL	RNA splicing	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Their specificity for RNA splicing instead of DNA is given by cytoplasmic proteins .
	manualset3
170143	3	413092	7	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Their specificity for RNA splicing instead of DNA is given by cytoplasmic proteins .
	manualset3
170144	4	413092	7	NULL	NULL	0	NULL	 cytoplasmic proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Their specificity for RNA splicing instead of DNA is given by cytoplasmic proteins .
	manualset3
170145	1	413093	7	NULL	NULL	0	NULL	Activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of adenylate cyclase in cultured fibroblasts by trypsin .
	manualset3
170146	2	413093	7	NULL	NULL	0	NULL	adenylate cyclase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of adenylate cyclase in cultured fibroblasts by trypsin .
	manualset3
170147	3	413093	7	NULL	NULL	0	NULL	cultured fibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of adenylate cyclase in cultured fibroblasts by trypsin .
	manualset3
170148	4	413093	7	NULL	NULL	0	NULL	trypsin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of adenylate cyclase in cultured fibroblasts by trypsin .
	manualset3
170149	1	413094	7	NULL	NULL	0	NULL	susceptibility 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Their susceptibility to the specific UL97 kinase inhibitor , maribavir , was also examined .
	manualset3
170150	2	413094	7	NULL	NULL	0	NULL	specific UL97 kinase inhibitor	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Their susceptibility to the specific UL97 kinase inhibitor , maribavir , was also examined .
	manualset3
170151	3	413094	7	NULL	NULL	0	NULL	maribavir	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Their susceptibility to the specific UL97 kinase inhibitor , maribavir , was also examined .
	manualset3
170152	1	413095	7	NULL	NULL	NULL	NULL	Themes	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Themes such as pain management and mechanism of breathing occur frequently ; however , there is a lack of up-to-date literature for the nurse to refer to .
	manualset3
170153	2	413095	7	NULL	NULL	0	NULL	pain management	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Themes such as pain management and mechanism of breathing occur frequently ; however , there is a lack of up-to-date literature for the nurse to refer to .
	manualset3
170154	3	413095	7	NULL	NULL	0	NULL	mechanism of breathing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Themes such as pain management and mechanism of breathing occur frequently ; however , there is a lack of up-to-date literature for the nurse to refer to .
	manualset3
170155	4	413095	7	NULL	NULL	0	NULL	lack	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Themes such as pain management and mechanism of breathing occur frequently ; however , there is a lack of up-to-date literature for the nurse to refer to .
	manualset3
170156	5	413095	7	NULL	NULL	0	NULL	up-to-date literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Themes such as pain management and mechanism of breathing occur frequently ; however , there is a lack of up-to-date literature for the nurse to refer to .
	manualset3
170157	6	413095	7	NULL	NULL	0	NULL	nurse	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Themes such as pain management and mechanism of breathing occur frequently ; however , there is a lack of up-to-date literature for the nurse to refer to .
	manualset3
170158	1	413096	7	NULL	NULL	0	NULL	 LASSO	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , LASSO was used to choose putative SNPs from the candidates identified in the first stage .
	manualset3
170159	2	413096	7	NULL	NULL	0	NULL	putative SNPs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , LASSO was used to choose putative SNPs from the candidates identified in the first stage .
	manualset3
170160	3	413096	7	NULL	NULL	0	NULL	candidates	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , LASSO was used to choose putative SNPs from the candidates identified in the first stage .
	manualset3
170161	4	413096	7	NULL	NULL	0	NULL	first stage	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , LASSO was used to choose putative SNPs from the candidates identified in the first stage .
	manualset3
170162	1	413097	7	NULL	NULL	0	NULL	 correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , the correlation between the prolongation of wave V latency and its reduction ratio ( % ) of amplitude was represented as a parabola .
	manualset3
170163	2	413097	7	NULL	NULL	0	NULL	prolongation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , the correlation between the prolongation of wave V latency and its reduction ratio ( % ) of amplitude was represented as a parabola .
	manualset3
170164	3	413097	7	NULL	NULL	0	NULL	wave V latency	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , the correlation between the prolongation of wave V latency and its reduction ratio ( % ) of amplitude was represented as a parabola .
	manualset3
170165	4	413097	7	NULL	NULL	0	NULL	reduction ratio ( % ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , the correlation between the prolongation of wave V latency and its reduction ratio ( % ) of amplitude was represented as a parabola .
	manualset3
170166	5	413097	7	NULL	NULL	0	NULL	amplitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , the correlation between the prolongation of wave V latency and its reduction ratio ( % ) of amplitude was represented as a parabola .
	manualset3
170167	6	413097	7	NULL	NULL	0	NULL	parabola	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , the correlation between the prolongation of wave V latency and its reduction ratio ( % ) of amplitude was represented as a parabola .
	manualset3
170168	1	413098	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , the results of recent studies have validated prophylactic implantations of these devices in primary prevention in the post-infarction period ( MADIT , MUSTT , MADIT II studies ) and have demonstrated the superiority of IAD over antiarrhythmic drug therapy in terms of global survival in patients with severe ventricular arrhythmias ( AVID , CIDS , CASH studies ) .
	manualset3
170169	2	413098	7	NULL	NULL	0	NULL	recent studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , the results of recent studies have validated prophylactic implantations of these devices in primary prevention in the post-infarction period ( MADIT , MUSTT , MADIT II studies ) and have demonstrated the superiority of IAD over antiarrhythmic drug therapy in terms of global survival in patients with severe ventricular arrhythmias ( AVID , CIDS , CASH studies ) .
	manualset3
170170	3	413098	7	NULL	NULL	0	NULL	prophylactic implantations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , the results of recent studies have validated prophylactic implantations of these devices in primary prevention in the post-infarction period ( MADIT , MUSTT , MADIT II studies ) and have demonstrated the superiority of IAD over antiarrhythmic drug therapy in terms of global survival in patients with severe ventricular arrhythmias ( AVID , CIDS , CASH studies ) .
	manualset3
170171	4	413098	7	NULL	NULL	0	NULL	devices	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , the results of recent studies have validated prophylactic implantations of these devices in primary prevention in the post-infarction period ( MADIT , MUSTT , MADIT II studies ) and have demonstrated the superiority of IAD over antiarrhythmic drug therapy in terms of global survival in patients with severe ventricular arrhythmias ( AVID , CIDS , CASH studies ) .
	manualset3
170172	5	413098	7	NULL	NULL	0	NULL	primary prevention	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , the results of recent studies have validated prophylactic implantations of these devices in primary prevention in the post-infarction period ( MADIT , MUSTT , MADIT II studies ) and have demonstrated the superiority of IAD over antiarrhythmic drug therapy in terms of global survival in patients with severe ventricular arrhythmias ( AVID , CIDS , CASH studies ) .
	manualset3
170173	6	413098	7	NULL	NULL	0	NULL	post-infarction period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , the results of recent studies have validated prophylactic implantations of these devices in primary prevention in the post-infarction period ( MADIT , MUSTT , MADIT II studies ) and have demonstrated the superiority of IAD over antiarrhythmic drug therapy in terms of global survival in patients with severe ventricular arrhythmias ( AVID , CIDS , CASH studies ) .
	manualset3
170174	7	413098	7	NULL	NULL	0	NULL	MADIT studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , the results of recent studies have validated prophylactic implantations of these devices in primary prevention in the post-infarction period ( MADIT , MUSTT , MADIT II studies ) and have demonstrated the superiority of IAD over antiarrhythmic drug therapy in terms of global survival in patients with severe ventricular arrhythmias ( AVID , CIDS , CASH studies ) .
	manualset3
170175	8	413098	7	NULL	NULL	0	NULL	MUSTT studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , the results of recent studies have validated prophylactic implantations of these devices in primary prevention in the post-infarction period ( MADIT , MUSTT , MADIT II studies ) and have demonstrated the superiority of IAD over antiarrhythmic drug therapy in terms of global survival in patients with severe ventricular arrhythmias ( AVID , CIDS , CASH studies ) .
	manualset3
170176	9	413098	7	NULL	NULL	0	NULL	MADIT II studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , the results of recent studies have validated prophylactic implantations of these devices in primary prevention in the post-infarction period ( MADIT , MUSTT , MADIT II studies ) and have demonstrated the superiority of IAD over antiarrhythmic drug therapy in terms of global survival in patients with severe ventricular arrhythmias ( AVID , CIDS , CASH studies ) .
	manualset3
170177	10	413098	7	NULL	NULL	0	NULL	superiority	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , the results of recent studies have validated prophylactic implantations of these devices in primary prevention in the post-infarction period ( MADIT , MUSTT , MADIT II studies ) and have demonstrated the superiority of IAD over antiarrhythmic drug therapy in terms of global survival in patients with severe ventricular arrhythmias ( AVID , CIDS , CASH studies ) .
	manualset3
170178	11	413098	7	NULL	NULL	0	NULL	IAD	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , the results of recent studies have validated prophylactic implantations of these devices in primary prevention in the post-infarction period ( MADIT , MUSTT , MADIT II studies ) and have demonstrated the superiority of IAD over antiarrhythmic drug therapy in terms of global survival in patients with severe ventricular arrhythmias ( AVID , CIDS , CASH studies ) .
	manualset3
170179	12	413098	7	NULL	NULL	0	NULL	antiarrhythmic drug therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , the results of recent studies have validated prophylactic implantations of these devices in primary prevention in the post-infarction period ( MADIT , MUSTT , MADIT II studies ) and have demonstrated the superiority of IAD over antiarrhythmic drug therapy in terms of global survival in patients with severe ventricular arrhythmias ( AVID , CIDS , CASH studies ) .
	manualset3
170180	13	413098	7	NULL	NULL	NULL	NULL	global survival	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Then , the results of recent studies have validated prophylactic implantations of these devices in primary prevention in the post-infarction period ( MADIT , MUSTT , MADIT II studies ) and have demonstrated the superiority of IAD over antiarrhythmic drug therapy in terms of global survival in patients with severe ventricular arrhythmias ( AVID , CIDS , CASH studies ) .
	manualset3
170181	14	413098	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , the results of recent studies have validated prophylactic implantations of these devices in primary prevention in the post-infarction period ( MADIT , MUSTT , MADIT II studies ) and have demonstrated the superiority of IAD over antiarrhythmic drug therapy in terms of global survival in patients with severe ventricular arrhythmias ( AVID , CIDS , CASH studies ) .
	manualset3
170182	15	413098	7	NULL	NULL	0	NULL	severe ventricular arrhythmias 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , the results of recent studies have validated prophylactic implantations of these devices in primary prevention in the post-infarction period ( MADIT , MUSTT , MADIT II studies ) and have demonstrated the superiority of IAD over antiarrhythmic drug therapy in terms of global survival in patients with severe ventricular arrhythmias ( AVID , CIDS , CASH studies ) .
	manualset3
170183	16	413098	7	NULL	NULL	NULL	NULL	AVID studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Then , the results of recent studies have validated prophylactic implantations of these devices in primary prevention in the post-infarction period ( MADIT , MUSTT , MADIT II studies ) and have demonstrated the superiority of IAD over antiarrhythmic drug therapy in terms of global survival in patients with severe ventricular arrhythmias ( AVID , CIDS , CASH studies ) .
	manualset3
170184	17	413098	7	NULL	NULL	0	NULL	CIDS studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , the results of recent studies have validated prophylactic implantations of these devices in primary prevention in the post-infarction period ( MADIT , MUSTT , MADIT II studies ) and have demonstrated the superiority of IAD over antiarrhythmic drug therapy in terms of global survival in patients with severe ventricular arrhythmias ( AVID , CIDS , CASH studies ) .
	manualset3
170185	18	413098	7	NULL	NULL	0	NULL	 CASH studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , the results of recent studies have validated prophylactic implantations of these devices in primary prevention in the post-infarction period ( MADIT , MUSTT , MADIT II studies ) and have demonstrated the superiority of IAD over antiarrhythmic drug therapy in terms of global survival in patients with severe ventricular arrhythmias ( AVID , CIDS , CASH studies ) .
	manualset3
170186	1	413099	7	NULL	NULL	0	NULL	series	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , using a series of transfer procedures , we demonstrate that correct recognition does not generalize to song bouts containing novel motifs from familiar singers .
	manualset3
170187	2	413099	7	NULL	NULL	0	NULL	transfer procedures 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , using a series of transfer procedures , we demonstrate that correct recognition does not generalize to song bouts containing novel motifs from familiar singers .
	manualset3
170188	3	413099	7	NULL	NULL	0	NULL	correct recognition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , using a series of transfer procedures , we demonstrate that correct recognition does not generalize to song bouts containing novel motifs from familiar singers .
	manualset3
170189	4	413099	7	NULL	NULL	0	NULL	song bouts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , using a series of transfer procedures , we demonstrate that correct recognition does not generalize to song bouts containing novel motifs from familiar singers .
	manualset3
170190	5	413099	7	NULL	NULL	0	NULL	 novel motifs	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , using a series of transfer procedures , we demonstrate that correct recognition does not generalize to song bouts containing novel motifs from familiar singers .
	manualset3
170191	6	413099	7	NULL	NULL	0	NULL	familiar singers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , using a series of transfer procedures , we demonstrate that correct recognition does not generalize to song bouts containing novel motifs from familiar singers .
	manualset3
170192	1	413100	7	NULL	NULL	0	NULL	symmetry	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , we hypothesize the symmetry , repulsion and attraction of NT EMF boxes : If a pair of NT EMF boxes are ( quasi ) mirror or complementary symmetric about a plane ( curve ) or point , they repulse or attract from each other because there is a repulsive or attractive EMF force between them .
	manualset3
170193	2	413100	7	NULL	NULL	0	NULL	 repulsion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , we hypothesize the symmetry , repulsion and attraction of NT EMF boxes : If a pair of NT EMF boxes are ( quasi ) mirror or complementary symmetric about a plane ( curve ) or point , they repulse or attract from each other because there is a repulsive or attractive EMF force between them .
	manualset3
170194	3	413100	7	NULL	NULL	0	NULL	attraction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , we hypothesize the symmetry , repulsion and attraction of NT EMF boxes : If a pair of NT EMF boxes are ( quasi ) mirror or complementary symmetric about a plane ( curve ) or point , they repulse or attract from each other because there is a repulsive or attractive EMF force between them .
	manualset3
170195	4	413100	7	NULL	NULL	0	NULL	NT EMF boxes	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , we hypothesize the symmetry , repulsion and attraction of NT EMF boxes : If a pair of NT EMF boxes are ( quasi ) mirror or complementary symmetric about a plane ( curve ) or point , they repulse or attract from each other because there is a repulsive or attractive EMF force between them .
	manualset3
170196	5	413100	7	NULL	NULL	0	NULL	pair	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , we hypothesize the symmetry , repulsion and attraction of NT EMF boxes : If a pair of NT EMF boxes are ( quasi ) mirror or complementary symmetric about a plane ( curve ) or point , they repulse or attract from each other because there is a repulsive or attractive EMF force between them .
	manualset3
170197	6	413100	7	NULL	NULL	0	NULL	NT EMF boxes	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , we hypothesize the symmetry , repulsion and attraction of NT EMF boxes : If a pair of NT EMF boxes are ( quasi ) mirror or complementary symmetric about a plane ( curve ) or point , they repulse or attract from each other because there is a repulsive or attractive EMF force between them .
	manualset3
170198	7	413100	7	NULL	NULL	0	NULL	( quasi ) mirror	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , we hypothesize the symmetry , repulsion and attraction of NT EMF boxes : If a pair of NT EMF boxes are ( quasi ) mirror or complementary symmetric about a plane ( curve ) or point , they repulse or attract from each other because there is a repulsive or attractive EMF force between them .
	manualset3
170199	8	413100	7	NULL	NULL	0	NULL	complementary symmetric	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , we hypothesize the symmetry , repulsion and attraction of NT EMF boxes : If a pair of NT EMF boxes are ( quasi ) mirror or complementary symmetric about a plane ( curve ) or point , they repulse or attract from each other because there is a repulsive or attractive EMF force between them .
	manualset3
170200	9	413100	7	NULL	NULL	0	NULL	plane ( curve )	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , we hypothesize the symmetry , repulsion and attraction of NT EMF boxes : If a pair of NT EMF boxes are ( quasi ) mirror or complementary symmetric about a plane ( curve ) or point , they repulse or attract from each other because there is a repulsive or attractive EMF force between them .
	manualset3
170201	10	413100	7	NULL	NULL	0	NULL	 point 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , we hypothesize the symmetry , repulsion and attraction of NT EMF boxes : If a pair of NT EMF boxes are ( quasi ) mirror or complementary symmetric about a plane ( curve ) or point , they repulse or attract from each other because there is a repulsive or attractive EMF force between them .
	manualset3
170204	13	413100	7	NULL	NULL	0	NULL	repulsive EMF force	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , we hypothesize the symmetry , repulsion and attraction of NT EMF boxes : If a pair of NT EMF boxes are ( quasi ) mirror or complementary symmetric about a plane ( curve ) or point , they repulse or attract from each other because there is a repulsive or attractive EMF force between them .
	manualset3
170205	14	413100	7	NULL	NULL	0	NULL	attractive EMF force 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Then , we hypothesize the symmetry , repulsion and attraction of NT EMF boxes : If a pair of NT EMF boxes are ( quasi ) mirror or complementary symmetric about a plane ( curve ) or point , they repulse or attract from each other because there is a repulsive or attractive EMF force between them .
	manualset3
170206	1	413101	7	NULL	NULL	0	NULL	non invasive investigations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Then follow non invasive investigations i.e. ergometry , myocardial radionuclide scan and a continuous ECG recording for 24 hours .
	manualset3
170207	2	413101	7	NULL	NULL	0	NULL	ergometry 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Then follow non invasive investigations i.e. ergometry , myocardial radionuclide scan and a continuous ECG recording for 24 hours .
	manualset3
170208	3	413101	7	NULL	NULL	0	NULL	myocardial radionuclide scan	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Then follow non invasive investigations i.e. ergometry , myocardial radionuclide scan and a continuous ECG recording for 24 hours .
	manualset3
170209	4	413101	7	NULL	NULL	0	NULL	 continuous ECG recording	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Then follow non invasive investigations i.e. ergometry , myocardial radionuclide scan and a continuous ECG recording for 24 hours .
	manualset3
170210	5	413101	7	NULL	NULL	0	NULL	 24 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Then follow non invasive investigations i.e. ergometry , myocardial radionuclide scan and a continuous ECG recording for 24 hours .
	manualset3
170211	1	413102	7	NULL	NULL	0	NULL	Activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of distinct multidrug-resistance ( P-glycoprotein ) genes during rat liver regeneration and hepatocarcinogenesis .
	manualset3
170212	2	413102	7	NULL	NULL	0	NULL	multidrug-resistance ( P-glycoprotein ) genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of distinct multidrug-resistance ( P-glycoprotein ) genes during rat liver regeneration and hepatocarcinogenesis .
	manualset3
170213	3	413102	7	NULL	NULL	0	NULL	rat liver regeneration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of distinct multidrug-resistance ( P-glycoprotein ) genes during rat liver regeneration and hepatocarcinogenesis .
	manualset3
170214	4	413102	7	NULL	NULL	0	NULL	hepatocarcinogenesis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of distinct multidrug-resistance ( P-glycoprotein ) genes during rat liver regeneration and hepatocarcinogenesis .
	manualset3
170216	1	413103	7	NULL	NULL	NULL	NULL	turn	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Then she gradually took a turn for the worse , particularly dementia became severer .
	manualset3
170217	2	413103	7	NULL	NULL	NULL	NULL	dementia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Then she gradually took a turn for the worse , particularly dementia became severer .
	manualset3
170218	1	413104	7	NULL	NULL	0	NULL	 linear stability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Then the linear stability , controllability , and observability of the system are investigated .
	manualset3
170219	2	413104	7	NULL	NULL	0	NULL	controllability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Then the linear stability , controllability , and observability of the system are investigated .
	manualset3
170220	3	413104	7	NULL	NULL	0	NULL	observability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Then the linear stability , controllability , and observability of the system are investigated .
	manualset3
170221	4	413104	7	NULL	NULL	0	NULL	system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Then the linear stability , controllability , and observability of the system are investigated .
	manualset3
170222	1	413105	7	NULL	NULL	0	NULL	differential proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Then these differential proteins were further identified by peptide mass fingerprint ( PMF ) and database search .
	manualset3
170223	2	413105	7	NULL	NULL	0	NULL	peptide mass fingerprint ( PMF ) search	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Then these differential proteins were further identified by peptide mass fingerprint ( PMF ) and database search .
	manualset3
170224	3	413105	7	NULL	NULL	0	NULL	database search	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Then these differential proteins were further identified by peptide mass fingerprint ( PMF ) and database search .
	manualset3
170225	1	413106	7	NULL	NULL	0	NULL	twelve years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Then twelve years later , in May 1982 , the Ministry of Health announced the outbreak of poliomyelitis in the parish of St. James , caused by the Type I virus .
	manualset3
170226	2	413106	7	NULL	NULL	0	NULL	May 1982	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Then twelve years later , in May 1982 , the Ministry of Health announced the outbreak of poliomyelitis in the parish of St. James , caused by the Type I virus .
	manualset3
170227	3	413106	7	NULL	NULL	0	NULL	Ministry of Health	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Then twelve years later , in May 1982 , the Ministry of Health announced the outbreak of poliomyelitis in the parish of St. James , caused by the Type I virus .
	manualset3
170228	4	413106	7	NULL	NULL	0	NULL	outbreak 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Then twelve years later , in May 1982 , the Ministry of Health announced the outbreak of poliomyelitis in the parish of St. James , caused by the Type I virus .
	manualset3
170229	5	413106	7	NULL	NULL	0	NULL	poliomyelitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Then twelve years later , in May 1982 , the Ministry of Health announced the outbreak of poliomyelitis in the parish of St. James , caused by the Type I virus .
	manualset3
170230	6	413106	7	NULL	NULL	0	NULL	 parish	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Then twelve years later , in May 1982 , the Ministry of Health announced the outbreak of poliomyelitis in the parish of St. James , caused by the Type I virus .
	manualset3
170231	7	413106	7	NULL	NULL	0	NULL	St. James	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Then twelve years later , in May 1982 , the Ministry of Health announced the outbreak of poliomyelitis in the parish of St. James , caused by the Type I virus .
	manualset3
170232	8	413106	7	NULL	NULL	0	NULL	Type I virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Then twelve years later , in May 1982 , the Ministry of Health announced the outbreak of poliomyelitis in the parish of St. James , caused by the Type I virus .
	manualset3
170233	1	413107	7	NULL	NULL	0	NULL	type I error probabilities	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Then type I error probabilities are not nominal , and the erroneous appearance of statistical significance can readily occur , particularly in large studies .
	manualset3
170234	2	413107	7	NULL	NULL	0	NULL	 nominal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Then type I error probabilities are not nominal , and the erroneous appearance of statistical significance can readily occur , particularly in large studies .
	manualset3
170235	3	413107	7	NULL	NULL	0	NULL	erroneous appearance	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Then type I error probabilities are not nominal , and the erroneous appearance of statistical significance can readily occur , particularly in large studies .
	manualset3
170236	4	413107	7	NULL	NULL	0	NULL	statistical significance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Then type I error probabilities are not nominal , and the erroneous appearance of statistical significance can readily occur , particularly in large studies .
	manualset3
170237	5	413107	7	NULL	NULL	0	NULL	 large studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Then type I error probabilities are not nominal , and the erroneous appearance of statistical significance can readily occur , particularly in large studies .
	manualset3
170238	1	413108	7	NULL	NULL	0	NULL	Theofylline	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Theofylline , an important drug in the treatment of severe bronchial asthma , increases urinary loss of magnesium .
	manualset3
170239	2	413108	7	NULL	NULL	0	NULL	 drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Theofylline , an important drug in the treatment of severe bronchial asthma , increases urinary loss of magnesium .
	manualset3
170240	3	413108	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Theofylline , an important drug in the treatment of severe bronchial asthma , increases urinary loss of magnesium .
	manualset3
170241	4	413108	7	NULL	NULL	0	NULL	severe bronchial asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Theofylline , an important drug in the treatment of severe bronchial asthma , increases urinary loss of magnesium .
	manualset3
170242	5	413108	7	NULL	NULL	0	NULL	urinary loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Theofylline , an important drug in the treatment of severe bronchial asthma , increases urinary loss of magnesium .
	manualset3
170243	6	413108	7	NULL	NULL	0	NULL	magnesium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Theofylline , an important drug in the treatment of severe bronchial asthma , increases urinary loss of magnesium .
	manualset3
170244	1	413109	7	NULL	NULL	0	NULL	Theoretical studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical and empirical studies of life history aim to account for resource allocation to the different components of fitness : survival , growth , and reproduction .
	manualset3
170245	2	413109	7	NULL	NULL	0	NULL	empirical studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical and empirical studies of life history aim to account for resource allocation to the different components of fitness : survival , growth , and reproduction .
	manualset3
170246	3	413109	7	NULL	NULL	0	NULL	life history	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical and empirical studies of life history aim to account for resource allocation to the different components of fitness : survival , growth , and reproduction .
	manualset3
170247	4	413109	7	NULL	NULL	0	NULL	resource allocation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical and empirical studies of life history aim to account for resource allocation to the different components of fitness : survival , growth , and reproduction .
	manualset3
170248	5	413109	7	NULL	NULL	0	NULL	different components	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical and empirical studies of life history aim to account for resource allocation to the different components of fitness : survival , growth , and reproduction .
	manualset3
170249	6	413109	7	NULL	NULL	0	NULL	 fitness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical and empirical studies of life history aim to account for resource allocation to the different components of fitness : survival , growth , and reproduction .
	manualset3
170250	7	413109	7	NULL	NULL	0	NULL	survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical and empirical studies of life history aim to account for resource allocation to the different components of fitness : survival , growth , and reproduction .
	manualset3
170251	8	413109	7	NULL	NULL	0	NULL	growth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical and empirical studies of life history aim to account for resource allocation to the different components of fitness : survival , growth , and reproduction .
	manualset3
170252	9	413109	7	NULL	NULL	0	NULL	reproduction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical and empirical studies of life history aim to account for resource allocation to the different components of fitness : survival , growth , and reproduction .
	manualset3
170253	1	413110	7	NULL	NULL	0	NULL	Theoretical analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical and experimental analyses revealed that RNA : m5C MTases share a number of features with either RNA : m5U MTases or DNA : m5C MTases , which suggested a tentative phylogenetic model of relationships between these three classes of 5-methylpyrimidine MTases .
	manualset3
170254	2	413110	7	NULL	NULL	0	NULL	experimental analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical and experimental analyses revealed that RNA : m5C MTases share a number of features with either RNA : m5U MTases or DNA : m5C MTases , which suggested a tentative phylogenetic model of relationships between these three classes of 5-methylpyrimidine MTases .
	manualset3
170255	3	413110	7	NULL	NULL	0	NULL	RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical and experimental analyses revealed that RNA : m5C MTases share a number of features with either RNA : m5U MTases or DNA : m5C MTases , which suggested a tentative phylogenetic model of relationships between these three classes of 5-methylpyrimidine MTases .
	manualset3
170256	4	413110	7	NULL	NULL	NULL	NULL	m5C MTases	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Theoretical and experimental analyses revealed that RNA : m5C MTases share a number of features with either RNA : m5U MTases or DNA : m5C MTases , which suggested a tentative phylogenetic model of relationships between these three classes of 5-methylpyrimidine MTases .
	manualset3
170257	5	413110	7	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical and experimental analyses revealed that RNA : m5C MTases share a number of features with either RNA : m5U MTases or DNA : m5C MTases , which suggested a tentative phylogenetic model of relationships between these three classes of 5-methylpyrimidine MTases .
	manualset3
170258	6	413110	7	NULL	NULL	0	NULL	features	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical and experimental analyses revealed that RNA : m5C MTases share a number of features with either RNA : m5U MTases or DNA : m5C MTases , which suggested a tentative phylogenetic model of relationships between these three classes of 5-methylpyrimidine MTases .
	manualset3
170259	7	413110	7	NULL	NULL	0	NULL	RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical and experimental analyses revealed that RNA : m5C MTases share a number of features with either RNA : m5U MTases or DNA : m5C MTases , which suggested a tentative phylogenetic model of relationships between these three classes of 5-methylpyrimidine MTases .
	manualset3
170260	8	413110	7	NULL	NULL	0	NULL	m5U MTases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical and experimental analyses revealed that RNA : m5C MTases share a number of features with either RNA : m5U MTases or DNA : m5C MTases , which suggested a tentative phylogenetic model of relationships between these three classes of 5-methylpyrimidine MTases .
	manualset3
170261	9	413110	7	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical and experimental analyses revealed that RNA : m5C MTases share a number of features with either RNA : m5U MTases or DNA : m5C MTases , which suggested a tentative phylogenetic model of relationships between these three classes of 5-methylpyrimidine MTases .
	manualset3
170262	10	413110	7	NULL	NULL	0	NULL	m5C MTases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical and experimental analyses revealed that RNA : m5C MTases share a number of features with either RNA : m5U MTases or DNA : m5C MTases , which suggested a tentative phylogenetic model of relationships between these three classes of 5-methylpyrimidine MTases .
	manualset3
170263	11	413110	7	NULL	NULL	0	NULL	tentative phylogenetic model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical and experimental analyses revealed that RNA : m5C MTases share a number of features with either RNA : m5U MTases or DNA : m5C MTases , which suggested a tentative phylogenetic model of relationships between these three classes of 5-methylpyrimidine MTases .
	manualset3
170264	12	413110	7	NULL	NULL	0	NULL	relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical and experimental analyses revealed that RNA : m5C MTases share a number of features with either RNA : m5U MTases or DNA : m5C MTases , which suggested a tentative phylogenetic model of relationships between these three classes of 5-methylpyrimidine MTases .
	manualset3
170265	13	413110	7	NULL	NULL	0	NULL	three classes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical and experimental analyses revealed that RNA : m5C MTases share a number of features with either RNA : m5U MTases or DNA : m5C MTases , which suggested a tentative phylogenetic model of relationships between these three classes of 5-methylpyrimidine MTases .
	manualset3
170266	14	413110	7	NULL	NULL	0	NULL	5-methylpyrimidine MTases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical and experimental analyses revealed that RNA : m5C MTases share a number of features with either RNA : m5U MTases or DNA : m5C MTases , which suggested a tentative phylogenetic model of relationships between these three classes of 5-methylpyrimidine MTases .
	manualset3
170267	1	413111	7	NULL	NULL	0	NULL	Activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of endogenous nucleases in mature sperm cells upon interaction with exogenous DNA .
	manualset3
170268	2	413111	7	NULL	NULL	0	NULL	endogenous nucleases	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of endogenous nucleases in mature sperm cells upon interaction with exogenous DNA .
	manualset3
170269	3	413111	7	NULL	NULL	0	NULL	mature sperm cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of endogenous nucleases in mature sperm cells upon interaction with exogenous DNA .
	manualset3
170270	4	413111	7	NULL	NULL	0	NULL	interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of endogenous nucleases in mature sperm cells upon interaction with exogenous DNA .
	manualset3
170271	5	413111	7	NULL	NULL	0	NULL	exogenous DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of endogenous nucleases in mature sperm cells upon interaction with exogenous DNA .
	manualset3
170272	1	413112	7	NULL	NULL	0	NULL	Theoretical calculations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical calculations are confronted with experimental data measured for complexation reactions between metallic forms of astatine ( At ( + ) and AtO ( + ) ) and inorganic ligands ( Cl ( - ) , Br ( - ) and SCN ( - ) ) .
	manualset3
170273	2	413112	7	NULL	NULL	0	NULL	experimental data	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical calculations are confronted with experimental data measured for complexation reactions between metallic forms of astatine ( At ( + ) and AtO ( + ) ) and inorganic ligands ( Cl ( - ) , Br ( - ) and SCN ( - ) ) .
	manualset3
170274	3	413112	7	NULL	NULL	0	NULL	complexation reactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical calculations are confronted with experimental data measured for complexation reactions between metallic forms of astatine ( At ( + ) and AtO ( + ) ) and inorganic ligands ( Cl ( - ) , Br ( - ) and SCN ( - ) ) .
	manualset3
170275	4	413112	7	NULL	NULL	0	NULL	metallic forms	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical calculations are confronted with experimental data measured for complexation reactions between metallic forms of astatine ( At ( + ) and AtO ( + ) ) and inorganic ligands ( Cl ( - ) , Br ( - ) and SCN ( - ) ) .
	manualset3
170276	5	413112	7	NULL	NULL	0	NULL	astatine ( At ( + ) and AtO ( + ) )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical calculations are confronted with experimental data measured for complexation reactions between metallic forms of astatine ( At ( + ) and AtO ( + ) ) and inorganic ligands ( Cl ( - ) , Br ( - ) and SCN ( - ) ) .
	manualset3
170277	6	413112	7	NULL	NULL	0	NULL	inorganic ligands	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical calculations are confronted with experimental data measured for complexation reactions between metallic forms of astatine ( At ( + ) and AtO ( + ) ) and inorganic ligands ( Cl ( - ) , Br ( - ) and SCN ( - ) ) .
	manualset3
170278	7	413112	7	NULL	NULL	0	NULL	( Cl ( - ) , Br ( - ) and SCN ( - ) )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical calculations are confronted with experimental data measured for complexation reactions between metallic forms of astatine ( At ( + ) and AtO ( + ) ) and inorganic ligands ( Cl ( - ) , Br ( - ) and SCN ( - ) ) .
	manualset3
170279	1	413113	7	NULL	NULL	0	NULL	Theoretical investigation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical investigation of the reaction of Mn + with ethylene oxide .
	manualset3
170280	2	413113	7	NULL	NULL	0	NULL	 reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical investigation of the reaction of Mn + with ethylene oxide .
	manualset3
170281	3	413113	7	NULL	NULL	0	NULL	Mn+	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical investigation of the reaction of Mn + with ethylene oxide .
	manualset3
170282	4	413113	7	NULL	NULL	0	NULL	ethylene oxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical investigation of the reaction of Mn + with ethylene oxide .
	manualset3
170283	1	413114	7	NULL	NULL	0	NULL	Theoretical models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical models have revealed that spatial structure can favor the co-evolution of punishment and cooperation , by allowing individuals to only play and compete with those in their immediate neighborhood .
	manualset3
170284	2	413114	7	NULL	NULL	0	NULL	spatial structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical models have revealed that spatial structure can favor the co-evolution of punishment and cooperation , by allowing individuals to only play and compete with those in their immediate neighborhood .
	manualset3
170285	3	413114	7	NULL	NULL	0	NULL	co-evolution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical models have revealed that spatial structure can favor the co-evolution of punishment and cooperation , by allowing individuals to only play and compete with those in their immediate neighborhood .
	manualset3
170286	4	413114	7	NULL	NULL	0	NULL	punishment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical models have revealed that spatial structure can favor the co-evolution of punishment and cooperation , by allowing individuals to only play and compete with those in their immediate neighborhood .
	manualset3
170287	5	413114	7	NULL	NULL	0	NULL	cooperation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical models have revealed that spatial structure can favor the co-evolution of punishment and cooperation , by allowing individuals to only play and compete with those in their immediate neighborhood .
	manualset3
170288	6	413114	7	NULL	NULL	0	NULL	individuals	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical models have revealed that spatial structure can favor the co-evolution of punishment and cooperation , by allowing individuals to only play and compete with those in their immediate neighborhood .
	manualset3
170290	8	413114	7	NULL	NULL	0	NULL	neighborhood	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical models have revealed that spatial structure can favor the co-evolution of punishment and cooperation , by allowing individuals to only play and compete with those in their immediate neighborhood .
	manualset3
170291	1	413115	7	NULL	NULL	0	NULL	Theoretical study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical study on the electronic structure and optical properties of carbazole -- dimesitylborane as bipolar fluorophores for nondoped blue OLEDs .
	manualset3
170292	2	413115	7	NULL	NULL	0	NULL	electronic structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical study on the electronic structure and optical properties of carbazole -- dimesitylborane as bipolar fluorophores for nondoped blue OLEDs .
	manualset3
170293	3	413115	7	NULL	NULL	0	NULL	optical properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical study on the electronic structure and optical properties of carbazole -- dimesitylborane as bipolar fluorophores for nondoped blue OLEDs .
	manualset3
170294	4	413115	7	NULL	NULL	0	NULL	carbazole -- dimesitylborane	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical study on the electronic structure and optical properties of carbazole -- dimesitylborane as bipolar fluorophores for nondoped blue OLEDs .
	manualset3
170295	5	413115	7	NULL	NULL	0	NULL	bipolar fluorophores	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical study on the electronic structure and optical properties of carbazole -- dimesitylborane as bipolar fluorophores for nondoped blue OLEDs .
	manualset3
170296	6	413115	7	NULL	NULL	NULL	NULL	nondoped blue OLEDs	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Theoretical study on the electronic structure and optical properties of carbazole -- dimesitylborane as bipolar fluorophores for nondoped blue OLEDs .
	manualset3
170297	1	413116	7	NULL	NULL	0	NULL	mortality rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretically the mortality rate of prostate cancer can be reduced by the prevention programs and by the improvements of treatment methods , but the ` earlier ' diagnosis is certainly an easier and less expensive strategy to achieve the same objective .
	manualset3
170298	2	413116	7	NULL	NULL	0	NULL	prostate cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretically the mortality rate of prostate cancer can be reduced by the prevention programs and by the improvements of treatment methods , but the ` earlier ' diagnosis is certainly an easier and less expensive strategy to achieve the same objective .
	manualset3
170299	3	413116	7	NULL	NULL	0	NULL	prevention programs 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretically the mortality rate of prostate cancer can be reduced by the prevention programs and by the improvements of treatment methods , but the ` earlier ' diagnosis is certainly an easier and less expensive strategy to achieve the same objective .
	manualset3
170300	4	413116	7	NULL	NULL	0	NULL	improvements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretically the mortality rate of prostate cancer can be reduced by the prevention programs and by the improvements of treatment methods , but the ` earlier ' diagnosis is certainly an easier and less expensive strategy to achieve the same objective .
	manualset3
170301	5	413116	7	NULL	NULL	0	NULL	treatment methods	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretically the mortality rate of prostate cancer can be reduced by the prevention programs and by the improvements of treatment methods , but the ` earlier ' diagnosis is certainly an easier and less expensive strategy to achieve the same objective .
	manualset3
170302	6	413116	7	NULL	NULL	0	NULL	 ` earlier ' diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretically the mortality rate of prostate cancer can be reduced by the prevention programs and by the improvements of treatment methods , but the ` earlier ' diagnosis is certainly an easier and less expensive strategy to achieve the same objective .
	manualset3
170303	7	413116	7	NULL	NULL	0	NULL	 less expensive strategy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretically the mortality rate of prostate cancer can be reduced by the prevention programs and by the improvements of treatment methods , but the ` earlier ' diagnosis is certainly an easier and less expensive strategy to achieve the same objective .
	manualset3
170304	8	413116	7	NULL	NULL	0	NULL	objective	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretically the mortality rate of prostate cancer can be reduced by the prevention programs and by the improvements of treatment methods , but the ` earlier ' diagnosis is certainly an easier and less expensive strategy to achieve the same objective .
	manualset3
170305	1	413117	7	NULL	NULL	0	NULL	urinary free corticosteroid excretion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretically urinary free corticosteroid excretion should be affected by renal function and this would make it a less sensitive index of hypercortisolemia .
	manualset3
170306	2	413117	7	NULL	NULL	0	NULL	renal function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretically urinary free corticosteroid excretion should be affected by renal function and this would make it a less sensitive index of hypercortisolemia .
	manualset3
170307	3	413117	7	NULL	NULL	0	NULL	 less sensitive index	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretically urinary free corticosteroid excretion should be affected by renal function and this would make it a less sensitive index of hypercortisolemia .
	manualset3
170308	4	413117	7	NULL	NULL	0	NULL	hypercortisolemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretically urinary free corticosteroid excretion should be affected by renal function and this would make it a less sensitive index of hypercortisolemia .
	manualset3
170310	1	413118	7	NULL	NULL	0	NULL	Theory for all and rehabilitation for the few ( with money )	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	Theory for all and rehabilitation for the few ( with money ) : who does our theory serve ?
	manualset3
170311	2	413118	7	NULL	NULL	0	NULL	theory 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Theory for all and rehabilitation for the few ( with money ) : who does our theory serve ?
	manualset3
170313	1	413119	7	NULL	NULL	0	NULL	Activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of granulocytes by anti-neutrophil cytoplasmic antibodies ( ANCA ) : a Fc gamma RII-dependent process .
	manualset3
170314	2	413119	7	NULL	NULL	0	NULL	granulocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of granulocytes by anti-neutrophil cytoplasmic antibodies ( ANCA ) : a Fc gamma RII-dependent process .
	manualset3
170315	3	413119	7	NULL	NULL	0	NULL	anti-neutrophil cytoplasmic antibodies ( ANCA )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of granulocytes by anti-neutrophil cytoplasmic antibodies ( ANCA ) : a Fc gamma RII-dependent process .
	manualset3
170316	4	413119	7	NULL	NULL	0	NULL	Fc gamma RII-dependent process	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of granulocytes by anti-neutrophil cytoplasmic antibodies ( ANCA ) : a Fc gamma RII-dependent process .
	manualset3
170317	1	413120	7	NULL	NULL	NULL	NULL	Therapeutic stem cell plasticity	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therapeutic stem cell plasticity orchestrates tissue plasticity .
	manualset3
170318	2	413120	7	NULL	NULL	NULL	NULL	tissue plasticity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therapeutic stem cell plasticity orchestrates tissue plasticity .
	manualset3
170319	1	413121	7	NULL	NULL	0	NULL	Therapies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapies targeting the RAS may represent a promising paradigm for the prevention and treatment of hepatic fibrosis in the setting of chronic liver disease .
	manualset3
170320	2	413121	7	NULL	NULL	0	NULL	RAS	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapies targeting the RAS may represent a promising paradigm for the prevention and treatment of hepatic fibrosis in the setting of chronic liver disease .
	manualset3
170321	3	413121	7	NULL	NULL	0	NULL	prevention	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapies targeting the RAS may represent a promising paradigm for the prevention and treatment of hepatic fibrosis in the setting of chronic liver disease .
	manualset3
170322	4	413121	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapies targeting the RAS may represent a promising paradigm for the prevention and treatment of hepatic fibrosis in the setting of chronic liver disease .
	manualset3
170323	5	413121	7	NULL	NULL	0	NULL	hepatic fibrosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapies targeting the RAS may represent a promising paradigm for the prevention and treatment of hepatic fibrosis in the setting of chronic liver disease .
	manualset3
170324	6	413121	7	NULL	NULL	0	NULL	setting	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapies targeting the RAS may represent a promising paradigm for the prevention and treatment of hepatic fibrosis in the setting of chronic liver disease .
	manualset3
170325	7	413121	7	NULL	NULL	0	NULL	chronic liver disease	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapies targeting the RAS may represent a promising paradigm for the prevention and treatment of hepatic fibrosis in the setting of chronic liver disease .
	manualset3
170326	1	413122	7	NULL	NULL	0	NULL	Therapy modifications	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy modifications in response to poorly controlled hypertension , dyslipidemia , and diabetes mellitus .
	manualset3
170327	2	413122	7	NULL	NULL	NULL	NULL	poorly controlled hypertension	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therapy modifications in response to poorly controlled hypertension , dyslipidemia , and diabetes mellitus .
	manualset3
170328	3	413122	7	NULL	NULL	NULL	NULL	dyslipidemia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therapy modifications in response to poorly controlled hypertension , dyslipidemia , and diabetes mellitus .
	manualset3
170329	4	413122	7	NULL	NULL	NULL	NULL	diabetes mellitus	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therapy modifications in response to poorly controlled hypertension , dyslipidemia , and diabetes mellitus .
	manualset3
171312	5	413122	7	NULL	NULL	0	NULL	response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy modifications in response to poorly controlled hypertension , dyslipidemia , and diabetes mellitus .
	manualset3
170330	1	413123	7	NULL	NULL	0	NULL	Therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy of HH depends primarily on the nature of the underlying condition .
	manualset3
170331	2	413123	7	NULL	NULL	0	NULL	HH	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy of HH depends primarily on the nature of the underlying condition .
	manualset3
170332	3	413123	7	NULL	NULL	0	NULL	 nature	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy of HH depends primarily on the nature of the underlying condition .
	manualset3
170333	4	413123	7	NULL	NULL	0	NULL	underlying condition	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy of HH depends primarily on the nature of the underlying condition .
	manualset3
170334	1	413124	7	NULL	NULL	0	NULL	Therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy of advanced prostate cancer with granulocyte macrophage colony-stimulating factor .
	manualset3
170335	2	413124	7	NULL	NULL	0	NULL	advanced prostate cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy of advanced prostate cancer with granulocyte macrophage colony-stimulating factor .
	manualset3
170336	3	413124	7	NULL	NULL	0	NULL	granulocyte macrophage colony-stimulating factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy of advanced prostate cancer with granulocyte macrophage colony-stimulating factor .
	manualset3
170337	1	413125	7	NULL	NULL	0	NULL	Therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy of chronic viral hepatitis .
	manualset3
170338	2	413125	7	NULL	NULL	0	NULL	chronic viral hepatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy of chronic viral hepatitis .
	manualset3
170339	1	413126	7	NULL	NULL	0	NULL	Activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of histamine H2-receptors by St 600 .
	manualset3
170340	2	413126	7	NULL	NULL	0	NULL	histamine H2-receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of histamine H2-receptors by St 600 .
	manualset3
170341	3	413126	7	NULL	NULL	0	NULL	St 600	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of histamine H2-receptors by St 600 .
	manualset3
170342	1	413127	7	NULL	NULL	0	NULL	Therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy was described and the correlates of antibiotic prescriptions in the previous year were identified using multivariate logistic regression .
	manualset3
170343	2	413127	7	NULL	NULL	0	NULL	antibiotic prescriptions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy was described and the correlates of antibiotic prescriptions in the previous year were identified using multivariate logistic regression .
	manualset3
170344	3	413127	7	NULL	NULL	0	NULL	previous year	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy was described and the correlates of antibiotic prescriptions in the previous year were identified using multivariate logistic regression .
	manualset3
170345	4	413127	7	NULL	NULL	0	NULL	multivariate logistic regression	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy was described and the correlates of antibiotic prescriptions in the previous year were identified using multivariate logistic regression .
	manualset3
170346	1	413128	7	NULL	NULL	0	NULL	Therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy with the CSD was associated with up-regulated mRNA expression for alpha-myosin heavy chain and down-regulated mRNA expression of A - and B - type natriuretic peptides , cytokines and favorably modulated cytoskeletal proteins .
	manualset3
170347	2	413128	7	NULL	NULL	0	NULL	 CSD	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy with the CSD was associated with up-regulated mRNA expression for alpha-myosin heavy chain and down-regulated mRNA expression of A - and B - type natriuretic peptides , cytokines and favorably modulated cytoskeletal proteins .
	manualset3
170348	3	413128	7	NULL	NULL	0	NULL	 up-regulated mRNA expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy with the CSD was associated with up-regulated mRNA expression for alpha-myosin heavy chain and down-regulated mRNA expression of A - and B - type natriuretic peptides , cytokines and favorably modulated cytoskeletal proteins .
	manualset3
170349	4	413128	7	NULL	NULL	0	NULL	alpha-myosin heavy chain 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy with the CSD was associated with up-regulated mRNA expression for alpha-myosin heavy chain and down-regulated mRNA expression of A - and B - type natriuretic peptides , cytokines and favorably modulated cytoskeletal proteins .
	manualset3
170350	5	413128	7	NULL	NULL	0	NULL	down-regulated mRNA expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy with the CSD was associated with up-regulated mRNA expression for alpha-myosin heavy chain and down-regulated mRNA expression of A - and B - type natriuretic peptides , cytokines and favorably modulated cytoskeletal proteins .
	manualset3
170351	6	413128	7	NULL	NULL	0	NULL	A -type natriuretic peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy with the CSD was associated with up-regulated mRNA expression for alpha-myosin heavy chain and down-regulated mRNA expression of A - and B - type natriuretic peptides , cytokines and favorably modulated cytoskeletal proteins .
	manualset3
170352	7	413128	7	NULL	NULL	0	NULL	B - type natriuretic peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy with the CSD was associated with up-regulated mRNA expression for alpha-myosin heavy chain and down-regulated mRNA expression of A - and B - type natriuretic peptides , cytokines and favorably modulated cytoskeletal proteins .
	manualset3
170353	8	413128	7	NULL	NULL	0	NULL	cytokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy with the CSD was associated with up-regulated mRNA expression for alpha-myosin heavy chain and down-regulated mRNA expression of A - and B - type natriuretic peptides , cytokines and favorably modulated cytoskeletal proteins .
	manualset3
170354	9	413128	7	NULL	NULL	0	NULL	cytoskeletal proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy with the CSD was associated with up-regulated mRNA expression for alpha-myosin heavy chain and down-regulated mRNA expression of A - and B - type natriuretic peptides , cytokines and favorably modulated cytoskeletal proteins .
	manualset3
170355	1	413129	7	NULL	NULL	0	NULL	Therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy with zidovudine may be partially responsible for these recent improvements .
	manualset3
170356	2	413129	7	NULL	NULL	0	NULL	zidovudine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy with zidovudine may be partially responsible for these recent improvements .
	manualset3
170357	3	413129	7	NULL	NULL	0	NULL	 improvements	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy with zidovudine may be partially responsible for these recent improvements .
	manualset3
170358	1	413130	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There also is evidence that activity during growth modulates the external geometry and trabecular architecture , potentially enhancing skeletal strength , while during the adult years activity may reduce age-related bone loss .
	manualset3
170359	2	413130	7	NULL	NULL	0	NULL	activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There also is evidence that activity during growth modulates the external geometry and trabecular architecture , potentially enhancing skeletal strength , while during the adult years activity may reduce age-related bone loss .
	manualset3
170360	3	413130	7	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There also is evidence that activity during growth modulates the external geometry and trabecular architecture , potentially enhancing skeletal strength , while during the adult years activity may reduce age-related bone loss .
	manualset3
170361	4	413130	7	NULL	NULL	0	NULL	external geometry	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There also is evidence that activity during growth modulates the external geometry and trabecular architecture , potentially enhancing skeletal strength , while during the adult years activity may reduce age-related bone loss .
	manualset3
170362	5	413130	7	NULL	NULL	0	NULL	trabecular architecture	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There also is evidence that activity during growth modulates the external geometry and trabecular architecture , potentially enhancing skeletal strength , while during the adult years activity may reduce age-related bone loss .
	manualset3
170363	6	413130	7	NULL	NULL	0	NULL	skeletal strength 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There also is evidence that activity during growth modulates the external geometry and trabecular architecture , potentially enhancing skeletal strength , while during the adult years activity may reduce age-related bone loss .
	manualset3
170364	7	413130	7	NULL	NULL	0	NULL	adult years	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	There also is evidence that activity during growth modulates the external geometry and trabecular architecture , potentially enhancing skeletal strength , while during the adult years activity may reduce age-related bone loss .
	manualset3
170365	8	413130	7	NULL	NULL	0	NULL	activity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There also is evidence that activity during growth modulates the external geometry and trabecular architecture , potentially enhancing skeletal strength , while during the adult years activity may reduce age-related bone loss .
	manualset3
170366	9	413130	7	NULL	NULL	0	NULL	age-related bone loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There also is evidence that activity during growth modulates the external geometry and trabecular architecture , potentially enhancing skeletal strength , while during the adult years activity may reduce age-related bone loss .
	manualset3
170377	1	413131	7	NULL	NULL	0	NULL	11 affected families	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There are 11 affected families with an average of 3.5 affected members per family , and a rate of occurrence consistent with autosomal dominant transmission .
	manualset3
170378	2	413131	7	NULL	NULL	0	NULL	average	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There are 11 affected families with an average of 3.5 affected members per family , and a rate of occurrence consistent with autosomal dominant transmission .
	manualset3
170379	3	413131	7	NULL	NULL	0	NULL	3.5 affected members per family	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There are 11 affected families with an average of 3.5 affected members per family , and a rate of occurrence consistent with autosomal dominant transmission .
	manualset3
170380	4	413131	7	NULL	NULL	0	NULL	rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There are 11 affected families with an average of 3.5 affected members per family , and a rate of occurrence consistent with autosomal dominant transmission .
	manualset3
170381	5	413131	7	NULL	NULL	0	NULL	 occurrence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There are 11 affected families with an average of 3.5 affected members per family , and a rate of occurrence consistent with autosomal dominant transmission .
	manualset3
170382	6	413131	7	NULL	NULL	NULL	NULL	autosomal dominant transmission	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There are 11 affected families with an average of 3.5 affected members per family , and a rate of occurrence consistent with autosomal dominant transmission .
	manualset3
170383	1	413132	7	NULL	NULL	0	NULL	three ryanodine receptor isoforms	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There are at least three ryanodine receptor isoforms in various tissues .
	manualset3
170384	2	413132	7	NULL	NULL	0	NULL	tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	There are at least three ryanodine receptor isoforms in various tissues .
	manualset3
170385	1	413133	7	NULL	NULL	0	NULL	basic principles	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	There are basic principles and techniques of measurement that are relevant across biomedical disciplines .
	manualset3
170386	2	413133	7	NULL	NULL	0	NULL	techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	There are basic principles and techniques of measurement that are relevant across biomedical disciplines .
	manualset3
170387	3	413133	7	NULL	NULL	0	NULL	measurement	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There are basic principles and techniques of measurement that are relevant across biomedical disciplines .
	manualset3
170388	4	413133	7	NULL	NULL	0	NULL	biomedical disciplines	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	There are basic principles and techniques of measurement that are relevant across biomedical disciplines .
	manualset3
170389	1	413134	7	NULL	NULL	0	NULL	Activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of multiple RTKs within individual GBMs provides a theoretical mechanism of resistance ; however , the spectrum of functional RTK dependence among tumor cell subpopulations in actual tumors is unknown .
	manualset3
170390	2	413134	7	NULL	NULL	0	NULL	multiple RTKs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of multiple RTKs within individual GBMs provides a theoretical mechanism of resistance ; however , the spectrum of functional RTK dependence among tumor cell subpopulations in actual tumors is unknown .
	manualset3
170391	3	413134	7	NULL	NULL	0	NULL	individual GBMs	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of multiple RTKs within individual GBMs provides a theoretical mechanism of resistance ; however , the spectrum of functional RTK dependence among tumor cell subpopulations in actual tumors is unknown .
	manualset3
170392	4	413134	7	NULL	NULL	NULL	NULL	theoretical mechanism	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Activation of multiple RTKs within individual GBMs provides a theoretical mechanism of resistance ; however , the spectrum of functional RTK dependence among tumor cell subpopulations in actual tumors is unknown .
	manualset3
170393	5	413134	7	NULL	NULL	0	NULL	resistance	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of multiple RTKs within individual GBMs provides a theoretical mechanism of resistance ; however , the spectrum of functional RTK dependence among tumor cell subpopulations in actual tumors is unknown .
	manualset3
170394	6	413134	7	NULL	NULL	0	NULL	spectrum	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of multiple RTKs within individual GBMs provides a theoretical mechanism of resistance ; however , the spectrum of functional RTK dependence among tumor cell subpopulations in actual tumors is unknown .
	manualset3
170395	7	413134	7	NULL	NULL	0	NULL	functional RTK	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of multiple RTKs within individual GBMs provides a theoretical mechanism of resistance ; however , the spectrum of functional RTK dependence among tumor cell subpopulations in actual tumors is unknown .
	manualset3
170396	8	413134	7	NULL	NULL	0	NULL	tumor cell subpopulations 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of multiple RTKs within individual GBMs provides a theoretical mechanism of resistance ; however , the spectrum of functional RTK dependence among tumor cell subpopulations in actual tumors is unknown .
	manualset3
170397	9	413134	7	NULL	NULL	0	NULL	actual tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of multiple RTKs within individual GBMs provides a theoretical mechanism of resistance ; however , the spectrum of functional RTK dependence among tumor cell subpopulations in actual tumors is unknown .
	manualset3
170398	1	413135	7	NULL	NULL	0	NULL	effective chemotherapeutic measures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There are currently no effective chemotherapeutic or biological control measures for PGD , which often peaks during the spring and fall when water temperatures are between 16-25 degrees C. The current diagnostic techniques of gross examination of gill clip wet mounts and histopathology are subject to false-negatives during the early stages of infection , and the quantifiable nature of end-point polymerase chain reaction ( PCR ) is subjective .
	manualset3
170399	2	413135	7	NULL	NULL	0	NULL	biological control measures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There are currently no effective chemotherapeutic or biological control measures for PGD , which often peaks during the spring and fall when water temperatures are between 16-25 degrees C. The current diagnostic techniques of gross examination of gill clip wet mounts and histopathology are subject to false-negatives during the early stages of infection , and the quantifiable nature of end-point polymerase chain reaction ( PCR ) is subjective .
	manualset3
170400	3	413135	7	NULL	NULL	0	NULL	PGD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There are currently no effective chemotherapeutic or biological control measures for PGD , which often peaks during the spring and fall when water temperatures are between 16-25 degrees C. The current diagnostic techniques of gross examination of gill clip wet mounts and histopathology are subject to false-negatives during the early stages of infection , and the quantifiable nature of end-point polymerase chain reaction ( PCR ) is subjective .
	manualset3
170401	4	413135	7	NULL	NULL	0	NULL	 spring 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	There are currently no effective chemotherapeutic or biological control measures for PGD , which often peaks during the spring and fall when water temperatures are between 16-25 degrees C. The current diagnostic techniques of gross examination of gill clip wet mounts and histopathology are subject to false-negatives during the early stages of infection , and the quantifiable nature of end-point polymerase chain reaction ( PCR ) is subjective .
	manualset3
170402	5	413135	7	NULL	NULL	0	NULL	 fall	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	There are currently no effective chemotherapeutic or biological control measures for PGD , which often peaks during the spring and fall when water temperatures are between 16-25 degrees C. The current diagnostic techniques of gross examination of gill clip wet mounts and histopathology are subject to false-negatives during the early stages of infection , and the quantifiable nature of end-point polymerase chain reaction ( PCR ) is subjective .
	manualset3
170403	6	413135	7	NULL	NULL	0	NULL	water temperatures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There are currently no effective chemotherapeutic or biological control measures for PGD , which often peaks during the spring and fall when water temperatures are between 16-25 degrees C. The current diagnostic techniques of gross examination of gill clip wet mounts and histopathology are subject to false-negatives during the early stages of infection , and the quantifiable nature of end-point polymerase chain reaction ( PCR ) is subjective .
	manualset3
170404	7	413135	7	NULL	NULL	0	NULL	16-25 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There are currently no effective chemotherapeutic or biological control measures for PGD , which often peaks during the spring and fall when water temperatures are between 16-25 degrees C. The current diagnostic techniques of gross examination of gill clip wet mounts and histopathology are subject to false-negatives during the early stages of infection , and the quantifiable nature of end-point polymerase chain reaction ( PCR ) is subjective .
	manualset3
170405	8	413135	7	NULL	NULL	0	NULL	current diagnostic techniques	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There are currently no effective chemotherapeutic or biological control measures for PGD , which often peaks during the spring and fall when water temperatures are between 16-25 degrees C. The current diagnostic techniques of gross examination of gill clip wet mounts and histopathology are subject to false-negatives during the early stages of infection , and the quantifiable nature of end-point polymerase chain reaction ( PCR ) is subjective .
	manualset3
170406	9	413135	7	NULL	NULL	0	NULL	gross examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There are currently no effective chemotherapeutic or biological control measures for PGD , which often peaks during the spring and fall when water temperatures are between 16-25 degrees C. The current diagnostic techniques of gross examination of gill clip wet mounts and histopathology are subject to false-negatives during the early stages of infection , and the quantifiable nature of end-point polymerase chain reaction ( PCR ) is subjective .
	manualset3
170407	10	413135	7	NULL	NULL	0	NULL	 gill clip wet mounts	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There are currently no effective chemotherapeutic or biological control measures for PGD , which often peaks during the spring and fall when water temperatures are between 16-25 degrees C. The current diagnostic techniques of gross examination of gill clip wet mounts and histopathology are subject to false-negatives during the early stages of infection , and the quantifiable nature of end-point polymerase chain reaction ( PCR ) is subjective .
	manualset3
170408	11	413135	7	NULL	NULL	0	NULL	histopathology	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There are currently no effective chemotherapeutic or biological control measures for PGD , which often peaks during the spring and fall when water temperatures are between 16-25 degrees C. The current diagnostic techniques of gross examination of gill clip wet mounts and histopathology are subject to false-negatives during the early stages of infection , and the quantifiable nature of end-point polymerase chain reaction ( PCR ) is subjective .
	manualset3
170409	12	413135	7	NULL	NULL	0	NULL	false-negatives	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There are currently no effective chemotherapeutic or biological control measures for PGD , which often peaks during the spring and fall when water temperatures are between 16-25 degrees C. The current diagnostic techniques of gross examination of gill clip wet mounts and histopathology are subject to false-negatives during the early stages of infection , and the quantifiable nature of end-point polymerase chain reaction ( PCR ) is subjective .
	manualset3
170410	13	413135	7	NULL	NULL	0	NULL	early stages of infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There are currently no effective chemotherapeutic or biological control measures for PGD , which often peaks during the spring and fall when water temperatures are between 16-25 degrees C. The current diagnostic techniques of gross examination of gill clip wet mounts and histopathology are subject to false-negatives during the early stages of infection , and the quantifiable nature of end-point polymerase chain reaction ( PCR ) is subjective .
	manualset3
170411	14	413135	7	NULL	NULL	0	NULL	quantifiable nature 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There are currently no effective chemotherapeutic or biological control measures for PGD , which often peaks during the spring and fall when water temperatures are between 16-25 degrees C. The current diagnostic techniques of gross examination of gill clip wet mounts and histopathology are subject to false-negatives during the early stages of infection , and the quantifiable nature of end-point polymerase chain reaction ( PCR ) is subjective .
	manualset3
170412	15	413135	7	NULL	NULL	0	NULL	end-point polymerase chain reaction ( PCR ) 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There are currently no effective chemotherapeutic or biological control measures for PGD , which often peaks during the spring and fall when water temperatures are between 16-25 degrees C. The current diagnostic techniques of gross examination of gill clip wet mounts and histopathology are subject to false-negatives during the early stages of infection , and the quantifiable nature of end-point polymerase chain reaction ( PCR ) is subjective .
	manualset3
170413	1	413136	7	NULL	NULL	0	NULL	different levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There are different levels of interaction between intracellular signals elicited by glucocorticoids and cytokines , with the final outcome being regulation of gene expression .
	manualset3
170414	2	413136	7	NULL	NULL	0	NULL	interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There are different levels of interaction between intracellular signals elicited by glucocorticoids and cytokines , with the final outcome being regulation of gene expression .
	manualset3
170415	3	413136	7	NULL	NULL	0	NULL	intracellular signals	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There are different levels of interaction between intracellular signals elicited by glucocorticoids and cytokines , with the final outcome being regulation of gene expression .
	manualset3
170416	4	413136	7	NULL	NULL	0	NULL	glucocorticoids 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There are different levels of interaction between intracellular signals elicited by glucocorticoids and cytokines , with the final outcome being regulation of gene expression .
	manualset3
170417	5	413136	7	NULL	NULL	0	NULL	cytokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There are different levels of interaction between intracellular signals elicited by glucocorticoids and cytokines , with the final outcome being regulation of gene expression .
	manualset3
170418	6	413136	7	NULL	NULL	0	NULL	 final outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There are different levels of interaction between intracellular signals elicited by glucocorticoids and cytokines , with the final outcome being regulation of gene expression .
	manualset3
170419	7	413136	7	NULL	NULL	0	NULL	regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There are different levels of interaction between intracellular signals elicited by glucocorticoids and cytokines , with the final outcome being regulation of gene expression .
	manualset3
170420	8	413136	7	NULL	NULL	0	NULL	 gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There are different levels of interaction between intracellular signals elicited by glucocorticoids and cytokines , with the final outcome being regulation of gene expression .
	manualset3
170421	1	413137	7	NULL	NULL	NULL	NULL	 early morning peak	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There are early morning peak and afternoon peak occurred in the diurnal variation , which are different from some metropolitans where only an afternoon peak is observed .
	manualset3
170422	2	413137	7	NULL	NULL	0	NULL	afternoon peak	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There are early morning peak and afternoon peak occurred in the diurnal variation , which are different from some metropolitans where only an afternoon peak is observed .
	manualset3
170423	3	413137	7	NULL	NULL	0	NULL	diurnal variation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There are early morning peak and afternoon peak occurred in the diurnal variation , which are different from some metropolitans where only an afternoon peak is observed .
	manualset3
170424	4	413137	7	NULL	NULL	0	NULL	metropolitans	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There are early morning peak and afternoon peak occurred in the diurnal variation , which are different from some metropolitans where only an afternoon peak is observed .
	manualset3
170425	5	413137	7	NULL	NULL	0	NULL	afternoon peak	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There are early morning peak and afternoon peak occurred in the diurnal variation , which are different from some metropolitans where only an afternoon peak is observed .
	manualset3
170426	1	413138	7	NULL	NULL	0	NULL	two types	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There are essentially two types of review : narrative reviews that follow no rules , exposing them to sampling error and bias ; and systematic reviews that attempt to minimize these effects by following an explicit structure for retrieving all of the evidence and attempting an objective synthesis of the results from the different trials .
	manualset3
170427	2	413138	7	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	There are essentially two types of review : narrative reviews that follow no rules , exposing them to sampling error and bias ; and systematic reviews that attempt to minimize these effects by following an explicit structure for retrieving all of the evidence and attempting an objective synthesis of the results from the different trials .
	manualset3
170428	3	413138	7	NULL	NULL	0	NULL	narrative reviews	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	There are essentially two types of review : narrative reviews that follow no rules , exposing them to sampling error and bias ; and systematic reviews that attempt to minimize these effects by following an explicit structure for retrieving all of the evidence and attempting an objective synthesis of the results from the different trials .
	manualset3
170429	4	413138	7	NULL	NULL	0	NULL	no rules	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There are essentially two types of review : narrative reviews that follow no rules , exposing them to sampling error and bias ; and systematic reviews that attempt to minimize these effects by following an explicit structure for retrieving all of the evidence and attempting an objective synthesis of the results from the different trials .
	manualset3
170430	5	413138	7	NULL	NULL	0	NULL	sampling error	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	There are essentially two types of review : narrative reviews that follow no rules , exposing them to sampling error and bias ; and systematic reviews that attempt to minimize these effects by following an explicit structure for retrieving all of the evidence and attempting an objective synthesis of the results from the different trials .
	manualset3
170431	6	413138	7	NULL	NULL	0	NULL	bias	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	There are essentially two types of review : narrative reviews that follow no rules , exposing them to sampling error and bias ; and systematic reviews that attempt to minimize these effects by following an explicit structure for retrieving all of the evidence and attempting an objective synthesis of the results from the different trials .
	manualset3
170432	7	413138	7	NULL	NULL	0	NULL	systematic reviews	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	There are essentially two types of review : narrative reviews that follow no rules , exposing them to sampling error and bias ; and systematic reviews that attempt to minimize these effects by following an explicit structure for retrieving all of the evidence and attempting an objective synthesis of the results from the different trials .
	manualset3
170433	8	413138	7	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There are essentially two types of review : narrative reviews that follow no rules , exposing them to sampling error and bias ; and systematic reviews that attempt to minimize these effects by following an explicit structure for retrieving all of the evidence and attempting an objective synthesis of the results from the different trials .
	manualset3
170434	9	413138	7	NULL	NULL	0	NULL	explicit structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There are essentially two types of review : narrative reviews that follow no rules , exposing them to sampling error and bias ; and systematic reviews that attempt to minimize these effects by following an explicit structure for retrieving all of the evidence and attempting an objective synthesis of the results from the different trials .
	manualset3
170435	10	413138	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There are essentially two types of review : narrative reviews that follow no rules , exposing them to sampling error and bias ; and systematic reviews that attempt to minimize these effects by following an explicit structure for retrieving all of the evidence and attempting an objective synthesis of the results from the different trials .
	manualset3
170436	11	413138	7	NULL	NULL	0	NULL	objective synthesis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There are essentially two types of review : narrative reviews that follow no rules , exposing them to sampling error and bias ; and systematic reviews that attempt to minimize these effects by following an explicit structure for retrieving all of the evidence and attempting an objective synthesis of the results from the different trials .
	manualset3
170437	12	413138	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There are essentially two types of review : narrative reviews that follow no rules , exposing them to sampling error and bias ; and systematic reviews that attempt to minimize these effects by following an explicit structure for retrieving all of the evidence and attempting an objective synthesis of the results from the different trials .
	manualset3
170438	13	413138	7	NULL	NULL	0	NULL	different trials	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There are essentially two types of review : narrative reviews that follow no rules , exposing them to sampling error and bias ; and systematic reviews that attempt to minimize these effects by following an explicit structure for retrieving all of the evidence and attempting an objective synthesis of the results from the different trials .
	manualset3
170439	1	413139	7	NULL	NULL	0	NULL	limited data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	There are extremely limited data on chlamydial sexually transmitted diseases ( STDs ) in many developing countries , including those in Central and South America .
	manualset3
170440	2	413139	7	NULL	NULL	0	NULL	chlamydial sexually transmitted diseases ( STDs )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There are extremely limited data on chlamydial sexually transmitted diseases ( STDs ) in many developing countries , including those in Central and South America .
	manualset3
170441	3	413139	7	NULL	NULL	0	NULL	developing countries	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	There are extremely limited data on chlamydial sexually transmitted diseases ( STDs ) in many developing countries , including those in Central and South America .
	manualset3
170442	4	413139	7	NULL	NULL	0	NULL	Central America	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	There are extremely limited data on chlamydial sexually transmitted diseases ( STDs ) in many developing countries , including those in Central and South America .
	manualset3
170443	5	413139	7	NULL	NULL	0	NULL	South America	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	There are extremely limited data on chlamydial sexually transmitted diseases ( STDs ) in many developing countries , including those in Central and South America .
	manualset3
170444	1	413140	7	NULL	NULL	0	NULL	few reports	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	There are few reports on hepatitis B e antigen ( HBeAg ) titers during nucleos ( t ) ide analogs treatment .
	manualset3
170445	2	413140	7	NULL	NULL	NULL	NULL	hepatitis B e antigen ( HBeAg ) titers	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There are few reports on hepatitis B e antigen ( HBeAg ) titers during nucleos ( t ) ide analogs treatment .
	manualset3
170446	3	413140	7	NULL	NULL	0	NULL	nucleos ( t ) ide analogs 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There are few reports on hepatitis B e antigen ( HBeAg ) titers during nucleos ( t ) ide analogs treatment .
	manualset3
170447	4	413140	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There are few reports on hepatitis B e antigen ( HBeAg ) titers during nucleos ( t ) ide analogs treatment .
	manualset3
170448	1	413141	7	NULL	NULL	0	NULL	four XacGSP molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	There are four XacGSP molecules in the crystal asymmetric unit .
	manualset3
170449	2	413141	7	NULL	NULL	0	NULL	crystal asymmetric unit	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There are four XacGSP molecules in the crystal asymmetric unit .
	manualset3
170450	1	413142	7	NULL	NULL	NULL	NULL	methods	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There are many methods available for estimation of insulin resistance which range from complex techniques down to simple indices .
	manualset3
170451	2	413142	7	NULL	NULL	0	NULL	estimation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	There are many methods available for estimation of insulin resistance which range from complex techniques down to simple indices .
	manualset3
170452	3	413142	7	NULL	NULL	NULL	NULL	insulin resistance	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There are many methods available for estimation of insulin resistance which range from complex techniques down to simple indices .
	manualset3
170453	4	413142	7	NULL	NULL	0	NULL	range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There are many methods available for estimation of insulin resistance which range from complex techniques down to simple indices .
	manualset3
170454	5	413142	7	NULL	NULL	0	NULL	complex techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	There are many methods available for estimation of insulin resistance which range from complex techniques down to simple indices .
	manualset3
170455	6	413142	7	NULL	NULL	0	NULL	simple indices	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There are many methods available for estimation of insulin resistance which range from complex techniques down to simple indices .
	manualset3
170456	1	413143	7	NULL	NULL	0	NULL	Activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of p34cdc2/cyclin B protein kinase requires dephosphorylation of p34cdc2 on Tyr15 .
	manualset3
170457	2	413143	7	NULL	NULL	0	NULL	p34cdc2/cyclin B protein kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of p34cdc2/cyclin B protein kinase requires dephosphorylation of p34cdc2 on Tyr15 .
	manualset3
170458	3	413143	7	NULL	NULL	0	NULL	dephosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of p34cdc2/cyclin B protein kinase requires dephosphorylation of p34cdc2 on Tyr15 .
	manualset3
170459	4	413143	7	NULL	NULL	0	NULL	 p34cdc2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of p34cdc2/cyclin B protein kinase requires dephosphorylation of p34cdc2 on Tyr15 .
	manualset3
170460	5	413143	7	NULL	NULL	0	NULL	Tyr15	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of p34cdc2/cyclin B protein kinase requires dephosphorylation of p34cdc2 on Tyr15 .
	manualset3
170461	1	413144	7	NULL	NULL	NULL	NULL	8 , 000 species 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There are more than 8 , 000 species of potential forest pests in China , including insects , plant diseases , rodents and lagomorphs , and hazardous plants .
	manualset3
170462	2	413144	7	NULL	NULL	0	NULL	potential forest pests	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	There are more than 8 , 000 species of potential forest pests in China , including insects , plant diseases , rodents and lagomorphs , and hazardous plants .
	manualset3
170463	3	413144	7	NULL	NULL	0	NULL	China	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	There are more than 8 , 000 species of potential forest pests in China , including insects , plant diseases , rodents and lagomorphs , and hazardous plants .
	manualset3
170464	4	413144	7	NULL	NULL	0	NULL	insects	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	There are more than 8 , 000 species of potential forest pests in China , including insects , plant diseases , rodents and lagomorphs , and hazardous plants .
	manualset3
170465	5	413144	7	NULL	NULL	0	NULL	plant diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There are more than 8 , 000 species of potential forest pests in China , including insects , plant diseases , rodents and lagomorphs , and hazardous plants .
	manualset3
170466	6	413144	7	NULL	NULL	0	NULL	 rodents	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	There are more than 8 , 000 species of potential forest pests in China , including insects , plant diseases , rodents and lagomorphs , and hazardous plants .
	manualset3
170467	7	413144	7	NULL	NULL	0	NULL	lagomorphs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	There are more than 8 , 000 species of potential forest pests in China , including insects , plant diseases , rodents and lagomorphs , and hazardous plants .
	manualset3
170468	8	413144	7	NULL	NULL	0	NULL	hazardous plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	There are more than 8 , 000 species of potential forest pests in China , including insects , plant diseases , rodents and lagomorphs , and hazardous plants .
	manualset3
170469	1	413145	7	NULL	NULL	0	NULL	multiple modalities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There are multiple modalities by which trauma occurs to the neck .
	manualset3
170470	2	413145	7	NULL	NULL	0	NULL	 trauma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There are multiple modalities by which trauma occurs to the neck .
	manualset3
170471	3	413145	7	NULL	NULL	0	NULL	neck	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There are multiple modalities by which trauma occurs to the neck .
	manualset3
170472	1	413146	7	NULL	NULL	0	NULL	no published national reports	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	There are no published national reports on hip fractures with large male samples , or on related inpatient mortality among veterans .
	manualset3
170473	2	413146	7	NULL	NULL	0	NULL	hip fractures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There are no published national reports on hip fractures with large male samples , or on related inpatient mortality among veterans .
	manualset3
170474	3	413146	7	NULL	NULL	0	NULL	large male samples	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There are no published national reports on hip fractures with large male samples , or on related inpatient mortality among veterans .
	manualset3
170475	4	413146	7	NULL	NULL	0	NULL	related inpatient mortality 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There are no published national reports on hip fractures with large male samples , or on related inpatient mortality among veterans .
	manualset3
170476	5	413146	7	NULL	NULL	0	NULL	veterans	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There are no published national reports on hip fractures with large male samples , or on related inpatient mortality among veterans .
	manualset3
170477	1	413147	7	NULL	NULL	0	NULL	 several factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There are several factors that contribute to the specificities of protein tyrosine kinases ( PTKs ) in signal transduction pathways .
	manualset3
170478	2	413147	7	NULL	NULL	0	NULL	specificities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There are several factors that contribute to the specificities of protein tyrosine kinases ( PTKs ) in signal transduction pathways .
	manualset3
170479	3	413147	7	NULL	NULL	0	NULL	protein tyrosine kinases ( PTKs )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There are several factors that contribute to the specificities of protein tyrosine kinases ( PTKs ) in signal transduction pathways .
	manualset3
170480	4	413147	7	NULL	NULL	0	NULL	 signal transduction pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There are several factors that contribute to the specificities of protein tyrosine kinases ( PTKs ) in signal transduction pathways .
	manualset3
170481	1	413148	7	NULL	NULL	0	NULL	 several thousand	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There are several thousand experienced registered nurses who meet the education requirements to be a nurse practitioner but who have not applied to the regulatory body for registration .
	manualset3
170482	2	413148	7	NULL	NULL	0	NULL	registered nurses	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There are several thousand experienced registered nurses who meet the education requirements to be a nurse practitioner but who have not applied to the regulatory body for registration .
	manualset3
170483	3	413148	7	NULL	NULL	0	NULL	education requirements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There are several thousand experienced registered nurses who meet the education requirements to be a nurse practitioner but who have not applied to the regulatory body for registration .
	manualset3
170484	4	413148	7	NULL	NULL	0	NULL	nurse practitioner	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	There are several thousand experienced registered nurses who meet the education requirements to be a nurse practitioner but who have not applied to the regulatory body for registration .
	manualset3
170485	5	413148	7	NULL	NULL	0	NULL	regulatory body	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	There are several thousand experienced registered nurses who meet the education requirements to be a nurse practitioner but who have not applied to the regulatory body for registration .
	manualset3
170486	6	413148	7	NULL	NULL	0	NULL	registration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There are several thousand experienced registered nurses who meet the education requirements to be a nurse practitioner but who have not applied to the regulatory body for registration .
	manualset3
170487	1	413149	7	NULL	NULL	0	NULL	Activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of the Wnt signaling pathway has been implicated recently in the pathogenesis of leukemia .
	manualset3
170488	2	413149	7	NULL	NULL	0	NULL	 Wnt signaling pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of the Wnt signaling pathway has been implicated recently in the pathogenesis of leukemia .
	manualset3
170489	3	413149	7	NULL	NULL	0	NULL	pathogenesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of the Wnt signaling pathway has been implicated recently in the pathogenesis of leukemia .
	manualset3
170490	4	413149	7	NULL	NULL	0	NULL	leukemia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of the Wnt signaling pathway has been implicated recently in the pathogenesis of leukemia .
	manualset3
170491	1	413150	7	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There are significant differences between the two structures in the extent of DNA bending , ligand conformation and groove binding .
	manualset3
170492	2	413150	7	NULL	NULL	0	NULL	 two structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There are significant differences between the two structures in the extent of DNA bending , ligand conformation and groove binding .
	manualset3
170493	3	413150	7	NULL	NULL	0	NULL	 extent	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There are significant differences between the two structures in the extent of DNA bending , ligand conformation and groove binding .
	manualset3
170494	4	413150	7	NULL	NULL	0	NULL	DNA bending	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There are significant differences between the two structures in the extent of DNA bending , ligand conformation and groove binding .
	manualset3
170495	5	413150	7	NULL	NULL	0	NULL	ligand conformation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There are significant differences between the two structures in the extent of DNA bending , ligand conformation and groove binding .
	manualset3
170496	6	413150	7	NULL	NULL	0	NULL	groove binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There are significant differences between the two structures in the extent of DNA bending , ligand conformation and groove binding .
	manualset3
170497	1	413151	7	NULL	NULL	0	NULL	three versions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There are three versions : one for outpatient facility-based , one for residential and one for home programs .
	manualset3
170498	2	413151	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There are three versions : one for outpatient facility-based , one for residential and one for home programs .
	manualset3
170499	3	413151	7	NULL	NULL	0	NULL	outpatient facility-based	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	There are three versions : one for outpatient facility-based , one for residential and one for home programs .
	manualset3
170500	4	413151	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There are three versions : one for outpatient facility-based , one for residential and one for home programs .
	manualset3
170501	5	413151	7	NULL	NULL	0	NULL	residential program	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	There are three versions : one for outpatient facility-based , one for residential and one for home programs .
	manualset3
170502	6	413151	7	NULL	NULL	0	NULL	 one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There are three versions : one for outpatient facility-based , one for residential and one for home programs .
	manualset3
170503	7	413151	7	NULL	NULL	0	NULL	home programs	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	There are three versions : one for outpatient facility-based , one for residential and one for home programs .
	manualset3
170504	1	413152	7	NULL	NULL	0	NULL	great variation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There has been great variation in the experimental and clinical procedures such as type of hypnotic intervention employed , the training of subjects and the timing of the intervention .
	manualset3
170505	2	413152	7	NULL	NULL	0	NULL	experimental procedure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There has been great variation in the experimental and clinical procedures such as type of hypnotic intervention employed , the training of subjects and the timing of the intervention .
	manualset3
170506	3	413152	7	NULL	NULL	0	NULL	clinical procedures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There has been great variation in the experimental and clinical procedures such as type of hypnotic intervention employed , the training of subjects and the timing of the intervention .
	manualset3
170507	4	413152	7	NULL	NULL	0	NULL	 type	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There has been great variation in the experimental and clinical procedures such as type of hypnotic intervention employed , the training of subjects and the timing of the intervention .
	manualset3
170508	5	413152	7	NULL	NULL	0	NULL	hypnotic intervention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There has been great variation in the experimental and clinical procedures such as type of hypnotic intervention employed , the training of subjects and the timing of the intervention .
	manualset3
170509	6	413152	7	NULL	NULL	0	NULL	training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There has been great variation in the experimental and clinical procedures such as type of hypnotic intervention employed , the training of subjects and the timing of the intervention .
	manualset3
170510	7	413152	7	NULL	NULL	0	NULL	subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There has been great variation in the experimental and clinical procedures such as type of hypnotic intervention employed , the training of subjects and the timing of the intervention .
	manualset3
170511	8	413152	7	NULL	NULL	NULL	NULL	 timing	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There has been great variation in the experimental and clinical procedures such as type of hypnotic intervention employed , the training of subjects and the timing of the intervention .
	manualset3
170512	9	413152	7	NULL	NULL	0	NULL	intervention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There has been great variation in the experimental and clinical procedures such as type of hypnotic intervention employed , the training of subjects and the timing of the intervention .
	manualset3
170513	1	413153	7	NULL	NULL	0	NULL	few reports	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	There have been few reports on the anti-angiogenic effects of low-dose cisplatin and hence the effect of low-dose metronomic ( LDM ) chemotherapy on the proliferation and neovascularization of H22 hepatocarcinoma cells is discussed in this research .
	manualset3
170514	2	413153	7	NULL	NULL	0	NULL	anti-angiogenic effects 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There have been few reports on the anti-angiogenic effects of low-dose cisplatin and hence the effect of low-dose metronomic ( LDM ) chemotherapy on the proliferation and neovascularization of H22 hepatocarcinoma cells is discussed in this research .
	manualset3
170515	3	413153	7	NULL	NULL	NULL	NULL	low-dose cisplatin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There have been few reports on the anti-angiogenic effects of low-dose cisplatin and hence the effect of low-dose metronomic ( LDM ) chemotherapy on the proliferation and neovascularization of H22 hepatocarcinoma cells is discussed in this research .
	manualset3
170516	4	413153	7	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There have been few reports on the anti-angiogenic effects of low-dose cisplatin and hence the effect of low-dose metronomic ( LDM ) chemotherapy on the proliferation and neovascularization of H22 hepatocarcinoma cells is discussed in this research .
	manualset3
170517	5	413153	7	NULL	NULL	NULL	NULL	low-dose metronomic ( LDM ) chemotherapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There have been few reports on the anti-angiogenic effects of low-dose cisplatin and hence the effect of low-dose metronomic ( LDM ) chemotherapy on the proliferation and neovascularization of H22 hepatocarcinoma cells is discussed in this research .
	manualset3
170518	6	413153	7	NULL	NULL	NULL	NULL	proliferation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There have been few reports on the anti-angiogenic effects of low-dose cisplatin and hence the effect of low-dose metronomic ( LDM ) chemotherapy on the proliferation and neovascularization of H22 hepatocarcinoma cells is discussed in this research .
	manualset3
170519	7	413153	7	NULL	NULL	0	NULL	neovascularization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There have been few reports on the anti-angiogenic effects of low-dose cisplatin and hence the effect of low-dose metronomic ( LDM ) chemotherapy on the proliferation and neovascularization of H22 hepatocarcinoma cells is discussed in this research .
	manualset3
170520	8	413153	7	NULL	NULL	0	NULL	H22 hepatocarcinoma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	There have been few reports on the anti-angiogenic effects of low-dose cisplatin and hence the effect of low-dose metronomic ( LDM ) chemotherapy on the proliferation and neovascularization of H22 hepatocarcinoma cells is discussed in this research .
	manualset3
170521	9	413153	7	NULL	NULL	0	NULL	 research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	There have been few reports on the anti-angiogenic effects of low-dose cisplatin and hence the effect of low-dose metronomic ( LDM ) chemotherapy on the proliferation and neovascularization of H22 hepatocarcinoma cells is discussed in this research .
	manualset3
170522	1	413154	7	NULL	NULL	0	NULL	neurologic events	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There have been no recurrent neurologic events , although two patients have died of complications of hemochromatosis .
	manualset3
170523	2	413154	7	NULL	NULL	0	NULL	two patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There have been no recurrent neurologic events , although two patients have died of complications of hemochromatosis .
	manualset3
170524	3	413154	7	NULL	NULL	0	NULL	 died of complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There have been no recurrent neurologic events , although two patients have died of complications of hemochromatosis .
	manualset3
170525	4	413154	7	NULL	NULL	0	NULL	hemochromatosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There have been no recurrent neurologic events , although two patients have died of complications of hemochromatosis .
	manualset3
170526	1	413155	7	NULL	NULL	0	NULL	Activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of the epidermal growth factor receptor ( EGFR ) seemed to underlie the ability of TPA to activate Akt as both PD153035 , an inhibitor of EGFR , and GW2974 , a dual-specific inhibitor of both EGFR and erbB2 , were able to effectively reduce TPA-induced Akt phosphorylation as well as TPA-stimulated EGFR and erbB2 tyrosine phosphorylation in a dose-dependent manner .
	manualset3
170527	2	413155	7	NULL	NULL	0	NULL	epidermal growth factor receptor ( EGFR )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of the epidermal growth factor receptor ( EGFR ) seemed to underlie the ability of TPA to activate Akt as both PD153035 , an inhibitor of EGFR , and GW2974 , a dual-specific inhibitor of both EGFR and erbB2 , were able to effectively reduce TPA-induced Akt phosphorylation as well as TPA-stimulated EGFR and erbB2 tyrosine phosphorylation in a dose-dependent manner .
	manualset3
170528	3	413155	7	NULL	NULL	0	NULL	ability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of the epidermal growth factor receptor ( EGFR ) seemed to underlie the ability of TPA to activate Akt as both PD153035 , an inhibitor of EGFR , and GW2974 , a dual-specific inhibitor of both EGFR and erbB2 , were able to effectively reduce TPA-induced Akt phosphorylation as well as TPA-stimulated EGFR and erbB2 tyrosine phosphorylation in a dose-dependent manner .
	manualset3
170529	4	413155	7	NULL	NULL	0	NULL	TPA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of the epidermal growth factor receptor ( EGFR ) seemed to underlie the ability of TPA to activate Akt as both PD153035 , an inhibitor of EGFR , and GW2974 , a dual-specific inhibitor of both EGFR and erbB2 , were able to effectively reduce TPA-induced Akt phosphorylation as well as TPA-stimulated EGFR and erbB2 tyrosine phosphorylation in a dose-dependent manner .
	manualset3
170530	5	413155	7	NULL	NULL	0	NULL	Akt	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of the epidermal growth factor receptor ( EGFR ) seemed to underlie the ability of TPA to activate Akt as both PD153035 , an inhibitor of EGFR , and GW2974 , a dual-specific inhibitor of both EGFR and erbB2 , were able to effectively reduce TPA-induced Akt phosphorylation as well as TPA-stimulated EGFR and erbB2 tyrosine phosphorylation in a dose-dependent manner .
	manualset3
170531	6	413155	7	NULL	NULL	0	NULL	PD153035	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of the epidermal growth factor receptor ( EGFR ) seemed to underlie the ability of TPA to activate Akt as both PD153035 , an inhibitor of EGFR , and GW2974 , a dual-specific inhibitor of both EGFR and erbB2 , were able to effectively reduce TPA-induced Akt phosphorylation as well as TPA-stimulated EGFR and erbB2 tyrosine phosphorylation in a dose-dependent manner .
	manualset3
170532	7	413155	7	NULL	NULL	0	NULL	inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of the epidermal growth factor receptor ( EGFR ) seemed to underlie the ability of TPA to activate Akt as both PD153035 , an inhibitor of EGFR , and GW2974 , a dual-specific inhibitor of both EGFR and erbB2 , were able to effectively reduce TPA-induced Akt phosphorylation as well as TPA-stimulated EGFR and erbB2 tyrosine phosphorylation in a dose-dependent manner .
	manualset3
170533	8	413155	7	NULL	NULL	0	NULL	EGFR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of the epidermal growth factor receptor ( EGFR ) seemed to underlie the ability of TPA to activate Akt as both PD153035 , an inhibitor of EGFR , and GW2974 , a dual-specific inhibitor of both EGFR and erbB2 , were able to effectively reduce TPA-induced Akt phosphorylation as well as TPA-stimulated EGFR and erbB2 tyrosine phosphorylation in a dose-dependent manner .
	manualset3
170534	9	413155	7	NULL	NULL	0	NULL	GW2974	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of the epidermal growth factor receptor ( EGFR ) seemed to underlie the ability of TPA to activate Akt as both PD153035 , an inhibitor of EGFR , and GW2974 , a dual-specific inhibitor of both EGFR and erbB2 , were able to effectively reduce TPA-induced Akt phosphorylation as well as TPA-stimulated EGFR and erbB2 tyrosine phosphorylation in a dose-dependent manner .
	manualset3
170535	10	413155	7	NULL	NULL	0	NULL	dual-specific inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of the epidermal growth factor receptor ( EGFR ) seemed to underlie the ability of TPA to activate Akt as both PD153035 , an inhibitor of EGFR , and GW2974 , a dual-specific inhibitor of both EGFR and erbB2 , were able to effectively reduce TPA-induced Akt phosphorylation as well as TPA-stimulated EGFR and erbB2 tyrosine phosphorylation in a dose-dependent manner .
	manualset3
170536	11	413155	7	NULL	NULL	0	NULL	EGFR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of the epidermal growth factor receptor ( EGFR ) seemed to underlie the ability of TPA to activate Akt as both PD153035 , an inhibitor of EGFR , and GW2974 , a dual-specific inhibitor of both EGFR and erbB2 , were able to effectively reduce TPA-induced Akt phosphorylation as well as TPA-stimulated EGFR and erbB2 tyrosine phosphorylation in a dose-dependent manner .
	manualset3
170537	12	413155	7	NULL	NULL	0	NULL	 erbB2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of the epidermal growth factor receptor ( EGFR ) seemed to underlie the ability of TPA to activate Akt as both PD153035 , an inhibitor of EGFR , and GW2974 , a dual-specific inhibitor of both EGFR and erbB2 , were able to effectively reduce TPA-induced Akt phosphorylation as well as TPA-stimulated EGFR and erbB2 tyrosine phosphorylation in a dose-dependent manner .
	manualset3
170538	13	413155	7	NULL	NULL	0	NULL	TPA-induced Akt phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of the epidermal growth factor receptor ( EGFR ) seemed to underlie the ability of TPA to activate Akt as both PD153035 , an inhibitor of EGFR , and GW2974 , a dual-specific inhibitor of both EGFR and erbB2 , were able to effectively reduce TPA-induced Akt phosphorylation as well as TPA-stimulated EGFR and erbB2 tyrosine phosphorylation in a dose-dependent manner .
	manualset3
170539	14	413155	7	NULL	NULL	0	NULL	TPA-stimulated EGFR	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of the epidermal growth factor receptor ( EGFR ) seemed to underlie the ability of TPA to activate Akt as both PD153035 , an inhibitor of EGFR , and GW2974 , a dual-specific inhibitor of both EGFR and erbB2 , were able to effectively reduce TPA-induced Akt phosphorylation as well as TPA-stimulated EGFR and erbB2 tyrosine phosphorylation in a dose-dependent manner .
	manualset3
170540	15	413155	7	NULL	NULL	0	NULL	erbB2 tyrosine phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of the epidermal growth factor receptor ( EGFR ) seemed to underlie the ability of TPA to activate Akt as both PD153035 , an inhibitor of EGFR , and GW2974 , a dual-specific inhibitor of both EGFR and erbB2 , were able to effectively reduce TPA-induced Akt phosphorylation as well as TPA-stimulated EGFR and erbB2 tyrosine phosphorylation in a dose-dependent manner .
	manualset3
170541	16	413155	7	NULL	NULL	0	NULL	dose-dependent manner	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of the epidermal growth factor receptor ( EGFR ) seemed to underlie the ability of TPA to activate Akt as both PD153035 , an inhibitor of EGFR , and GW2974 , a dual-specific inhibitor of both EGFR and erbB2 , were able to effectively reduce TPA-induced Akt phosphorylation as well as TPA-stimulated EGFR and erbB2 tyrosine phosphorylation in a dose-dependent manner .
	manualset3
170542	1	413156	7	NULL	NULL	0	NULL	growing realisation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a growing realisation that bipolar disorder represents a major , largely unmet , international public health challenge and that innovative methods for carrying out reliable and generalisable long-term pharmacological treatment trials , alone and in combination with cost-effective psychosocial and rehabilitative interventions , are urgently required .
	manualset3
170543	2	413156	7	NULL	NULL	NULL	NULL	bipolar disorder	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There is a growing realisation that bipolar disorder represents a major , largely unmet , international public health challenge and that innovative methods for carrying out reliable and generalisable long-term pharmacological treatment trials , alone and in combination with cost-effective psychosocial and rehabilitative interventions , are urgently required .
	manualset3
170544	3	413156	7	NULL	NULL	0	NULL	major , largely unmet , international public health challenge	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a growing realisation that bipolar disorder represents a major , largely unmet , international public health challenge and that innovative methods for carrying out reliable and generalisable long-term pharmacological treatment trials , alone and in combination with cost-effective psychosocial and rehabilitative interventions , are urgently required .
	manualset3
170545	4	413156	7	NULL	NULL	0	NULL	 innovative methods	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a growing realisation that bipolar disorder represents a major , largely unmet , international public health challenge and that innovative methods for carrying out reliable and generalisable long-term pharmacological treatment trials , alone and in combination with cost-effective psychosocial and rehabilitative interventions , are urgently required .
	manualset3
170546	5	413156	7	NULL	NULL	0	NULL	reliable and generalisable long-term pharmacological treatment trials	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a growing realisation that bipolar disorder represents a major , largely unmet , international public health challenge and that innovative methods for carrying out reliable and generalisable long-term pharmacological treatment trials , alone and in combination with cost-effective psychosocial and rehabilitative interventions , are urgently required .
	manualset3
170547	6	413156	7	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a growing realisation that bipolar disorder represents a major , largely unmet , international public health challenge and that innovative methods for carrying out reliable and generalisable long-term pharmacological treatment trials , alone and in combination with cost-effective psychosocial and rehabilitative interventions , are urgently required .
	manualset3
170548	7	413156	7	NULL	NULL	NULL	NULL	 cost-effective psychosocial interventions	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There is a growing realisation that bipolar disorder represents a major , largely unmet , international public health challenge and that innovative methods for carrying out reliable and generalisable long-term pharmacological treatment trials , alone and in combination with cost-effective psychosocial and rehabilitative interventions , are urgently required .
	manualset3
170549	8	413156	7	NULL	NULL	0	NULL	rehabilitative interventions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a growing realisation that bipolar disorder represents a major , largely unmet , international public health challenge and that innovative methods for carrying out reliable and generalisable long-term pharmacological treatment trials , alone and in combination with cost-effective psychosocial and rehabilitative interventions , are urgently required .
	manualset3
170550	1	413157	7	NULL	NULL	0	NULL	high correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a high correlation between the specificity of the mutant phenotype and the accumulation of transcripts in the presumptive distal regions of the cuticle-forming epithelial cells of the affected discs ; it is , in fact , the first gene reported whose expression is localized with respect to the proximo distal-forming axis .
	manualset3
170551	2	413157	7	NULL	NULL	0	NULL	specificity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a high correlation between the specificity of the mutant phenotype and the accumulation of transcripts in the presumptive distal regions of the cuticle-forming epithelial cells of the affected discs ; it is , in fact , the first gene reported whose expression is localized with respect to the proximo distal-forming axis .
	manualset3
170552	3	413157	7	NULL	NULL	0	NULL	mutant phenotype	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a high correlation between the specificity of the mutant phenotype and the accumulation of transcripts in the presumptive distal regions of the cuticle-forming epithelial cells of the affected discs ; it is , in fact , the first gene reported whose expression is localized with respect to the proximo distal-forming axis .
	manualset3
170553	4	413157	7	NULL	NULL	0	NULL	accumulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a high correlation between the specificity of the mutant phenotype and the accumulation of transcripts in the presumptive distal regions of the cuticle-forming epithelial cells of the affected discs ; it is , in fact , the first gene reported whose expression is localized with respect to the proximo distal-forming axis .
	manualset3
170554	5	413157	7	NULL	NULL	0	NULL	transcripts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a high correlation between the specificity of the mutant phenotype and the accumulation of transcripts in the presumptive distal regions of the cuticle-forming epithelial cells of the affected discs ; it is , in fact , the first gene reported whose expression is localized with respect to the proximo distal-forming axis .
	manualset3
170555	6	413157	7	NULL	NULL	0	NULL	presumptive distal regions	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a high correlation between the specificity of the mutant phenotype and the accumulation of transcripts in the presumptive distal regions of the cuticle-forming epithelial cells of the affected discs ; it is , in fact , the first gene reported whose expression is localized with respect to the proximo distal-forming axis .
	manualset3
170556	7	413157	7	NULL	NULL	0	NULL	cuticle-forming epithelial cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a high correlation between the specificity of the mutant phenotype and the accumulation of transcripts in the presumptive distal regions of the cuticle-forming epithelial cells of the affected discs ; it is , in fact , the first gene reported whose expression is localized with respect to the proximo distal-forming axis .
	manualset3
170557	8	413157	7	NULL	NULL	0	NULL	discs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a high correlation between the specificity of the mutant phenotype and the accumulation of transcripts in the presumptive distal regions of the cuticle-forming epithelial cells of the affected discs ; it is , in fact , the first gene reported whose expression is localized with respect to the proximo distal-forming axis .
	manualset3
170558	9	413157	7	NULL	NULL	0	NULL	first gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a high correlation between the specificity of the mutant phenotype and the accumulation of transcripts in the presumptive distal regions of the cuticle-forming epithelial cells of the affected discs ; it is , in fact , the first gene reported whose expression is localized with respect to the proximo distal-forming axis .
	manualset3
170559	10	413157	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a high correlation between the specificity of the mutant phenotype and the accumulation of transcripts in the presumptive distal regions of the cuticle-forming epithelial cells of the affected discs ; it is , in fact , the first gene reported whose expression is localized with respect to the proximo distal-forming axis .
	manualset3
170560	11	413157	7	NULL	NULL	0	NULL	proximo distal-forming axis	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a high correlation between the specificity of the mutant phenotype and the accumulation of transcripts in the presumptive distal regions of the cuticle-forming epithelial cells of the affected discs ; it is , in fact , the first gene reported whose expression is localized with respect to the proximo distal-forming axis .
	manualset3
170561	1	413158	7	NULL	NULL	0	NULL	amendments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a need here for amendments to be made to EU legislation , as currently nanoforms do not represent a separate category of substance in their own right .
	manualset3
170562	2	413158	7	NULL	NULL	0	NULL	EU legislation	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a need here for amendments to be made to EU legislation , as currently nanoforms do not represent a separate category of substance in their own right .
	manualset3
170563	3	413158	7	NULL	NULL	0	NULL	nanoforms	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a need here for amendments to be made to EU legislation , as currently nanoforms do not represent a separate category of substance in their own right .
	manualset3
170564	4	413158	7	NULL	NULL	0	NULL	separate category	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a need here for amendments to be made to EU legislation , as currently nanoforms do not represent a separate category of substance in their own right .
	manualset3
170565	5	413158	7	NULL	NULL	0	NULL	substance	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a need here for amendments to be made to EU legislation , as currently nanoforms do not represent a separate category of substance in their own right .
	manualset3
170566	1	413159	7	NULL	NULL	0	NULL	need 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a need to target these beliefs and self-efficacy expectations in health education and STD counselling and for more research to evaluate the psychosocial determinants of sexual partner referral quantitatively .
	manualset3
170567	2	413159	7	NULL	NULL	0	NULL	beliefs 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a need to target these beliefs and self-efficacy expectations in health education and STD counselling and for more research to evaluate the psychosocial determinants of sexual partner referral quantitatively .
	manualset3
170568	3	413159	7	NULL	NULL	0	NULL	self-efficacy expectations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a need to target these beliefs and self-efficacy expectations in health education and STD counselling and for more research to evaluate the psychosocial determinants of sexual partner referral quantitatively .
	manualset3
170569	4	413159	7	NULL	NULL	0	NULL	health education	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a need to target these beliefs and self-efficacy expectations in health education and STD counselling and for more research to evaluate the psychosocial determinants of sexual partner referral quantitatively .
	manualset3
170570	5	413159	7	NULL	NULL	0	NULL	STD counselling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a need to target these beliefs and self-efficacy expectations in health education and STD counselling and for more research to evaluate the psychosocial determinants of sexual partner referral quantitatively .
	manualset3
170571	6	413159	7	NULL	NULL	0	NULL	 research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a need to target these beliefs and self-efficacy expectations in health education and STD counselling and for more research to evaluate the psychosocial determinants of sexual partner referral quantitatively .
	manualset3
170572	7	413159	7	NULL	NULL	0	NULL	 psychosocial determinants	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a need to target these beliefs and self-efficacy expectations in health education and STD counselling and for more research to evaluate the psychosocial determinants of sexual partner referral quantitatively .
	manualset3
170573	8	413159	7	NULL	NULL	0	NULL	sexual partner referral	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a need to target these beliefs and self-efficacy expectations in health education and STD counselling and for more research to evaluate the psychosocial determinants of sexual partner referral quantitatively .
	manualset3
170575	1	413160	7	NULL	NULL	0	NULL	short section	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a short section on family planning , followed by a description of abortion legislation and its effects on the birth rate .
	manualset3
170576	2	413160	7	NULL	NULL	0	NULL	family planning	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a short section on family planning , followed by a description of abortion legislation and its effects on the birth rate .
	manualset3
170577	3	413160	7	NULL	NULL	0	NULL	description	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a short section on family planning , followed by a description of abortion legislation and its effects on the birth rate .
	manualset3
170578	4	413160	7	NULL	NULL	0	NULL	abortion legislation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a short section on family planning , followed by a description of abortion legislation and its effects on the birth rate .
	manualset3
170579	5	413160	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a short section on family planning , followed by a description of abortion legislation and its effects on the birth rate .
	manualset3
170580	6	413160	7	NULL	NULL	0	NULL	birth rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There is a short section on family planning , followed by a description of abortion legislation and its effects on the birth rate .
	manualset3
170581	1	413161	7	NULL	NULL	NULL	NULL	Activation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Activation of the immune system normally leads to removal of microbial pathogens , and after resolution of the inflammation immune homeostasis is restored .
	manualset3
170582	2	413161	7	NULL	NULL	0	NULL	immune system 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of the immune system normally leads to removal of microbial pathogens , and after resolution of the inflammation immune homeostasis is restored .
	manualset3
170583	3	413161	7	NULL	NULL	NULL	NULL	 removal	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Activation of the immune system normally leads to removal of microbial pathogens , and after resolution of the inflammation immune homeostasis is restored .
	manualset3
170584	4	413161	7	NULL	NULL	0	NULL	microbial pathogens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of the immune system normally leads to removal of microbial pathogens , and after resolution of the inflammation immune homeostasis is restored .
	manualset3
170585	5	413161	7	NULL	NULL	NULL	NULL	resolution	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Activation of the immune system normally leads to removal of microbial pathogens , and after resolution of the inflammation immune homeostasis is restored .
	manualset3
170586	6	413161	7	NULL	NULL	0	NULL	inflammation immune homeostasis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of the immune system normally leads to removal of microbial pathogens , and after resolution of the inflammation immune homeostasis is restored .
	manualset3
170587	1	413162	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is also evidence in support of integrating regular surveillance for upper-body morbidity into the routine care provided to women with breast cancer , with early diagnosis potentially contributing to more effective management and prevention of progression of these conditions .
	manualset3
170588	2	413162	7	NULL	NULL	0	NULL	support	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is also evidence in support of integrating regular surveillance for upper-body morbidity into the routine care provided to women with breast cancer , with early diagnosis potentially contributing to more effective management and prevention of progression of these conditions .
	manualset3
170589	3	413162	7	NULL	NULL	NULL	NULL	 regular surveillance	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There is also evidence in support of integrating regular surveillance for upper-body morbidity into the routine care provided to women with breast cancer , with early diagnosis potentially contributing to more effective management and prevention of progression of these conditions .
	manualset3
170590	4	413162	7	NULL	NULL	0	NULL	upper-body morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is also evidence in support of integrating regular surveillance for upper-body morbidity into the routine care provided to women with breast cancer , with early diagnosis potentially contributing to more effective management and prevention of progression of these conditions .
	manualset3
170591	5	413162	7	NULL	NULL	NULL	NULL	 routine care	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There is also evidence in support of integrating regular surveillance for upper-body morbidity into the routine care provided to women with breast cancer , with early diagnosis potentially contributing to more effective management and prevention of progression of these conditions .
	manualset3
170592	6	413162	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There is also evidence in support of integrating regular surveillance for upper-body morbidity into the routine care provided to women with breast cancer , with early diagnosis potentially contributing to more effective management and prevention of progression of these conditions .
	manualset3
170593	7	413162	7	NULL	NULL	0	NULL	breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There is also evidence in support of integrating regular surveillance for upper-body morbidity into the routine care provided to women with breast cancer , with early diagnosis potentially contributing to more effective management and prevention of progression of these conditions .
	manualset3
170594	8	413162	7	NULL	NULL	0	NULL	early diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is also evidence in support of integrating regular surveillance for upper-body morbidity into the routine care provided to women with breast cancer , with early diagnosis potentially contributing to more effective management and prevention of progression of these conditions .
	manualset3
170595	9	413162	7	NULL	NULL	0	NULL	 effective management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is also evidence in support of integrating regular surveillance for upper-body morbidity into the routine care provided to women with breast cancer , with early diagnosis potentially contributing to more effective management and prevention of progression of these conditions .
	manualset3
170596	10	413162	7	NULL	NULL	0	NULL	prevention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is also evidence in support of integrating regular surveillance for upper-body morbidity into the routine care provided to women with breast cancer , with early diagnosis potentially contributing to more effective management and prevention of progression of these conditions .
	manualset3
170597	11	413162	7	NULL	NULL	0	NULL	progression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There is also evidence in support of integrating regular surveillance for upper-body morbidity into the routine care provided to women with breast cancer , with early diagnosis potentially contributing to more effective management and prevention of progression of these conditions .
	manualset3
170598	12	413162	7	NULL	NULL	NULL	NULL	conditions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There is also evidence in support of integrating regular surveillance for upper-body morbidity into the routine care provided to women with breast cancer , with early diagnosis potentially contributing to more effective management and prevention of progression of these conditions .
	manualset3
170599	1	413163	7	NULL	NULL	0	NULL	need	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is also the need for a validated tool to assess pain in younger children .
	manualset3
170600	2	413163	7	NULL	NULL	0	NULL	validated tool	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	There is also the need for a validated tool to assess pain in younger children .
	manualset3
170601	3	413163	7	NULL	NULL	0	NULL	pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is also the need for a validated tool to assess pain in younger children .
	manualset3
170602	4	413163	7	NULL	NULL	0	NULL	younger children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There is also the need for a validated tool to assess pain in younger children .
	manualset3
170603	1	413164	7	NULL	NULL	0	NULL	 increase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There is an increase in oxygen uptake by the isolated mitochondria together with an increase in the specific surface of cristae .
	manualset3
170604	2	413164	7	NULL	NULL	0	NULL	oxygen uptake	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There is an increase in oxygen uptake by the isolated mitochondria together with an increase in the specific surface of cristae .
	manualset3
170605	3	413164	7	NULL	NULL	0	NULL	isolated mitochondria	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	There is an increase in oxygen uptake by the isolated mitochondria together with an increase in the specific surface of cristae .
	manualset3
170606	4	413164	7	NULL	NULL	0	NULL	 increase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There is an increase in oxygen uptake by the isolated mitochondria together with an increase in the specific surface of cristae .
	manualset3
170607	5	413164	7	NULL	NULL	0	NULL	 specific surface 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	There is an increase in oxygen uptake by the isolated mitochondria together with an increase in the specific surface of cristae .
	manualset3
170608	6	413164	7	NULL	NULL	0	NULL	cristae	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	There is an increase in oxygen uptake by the isolated mitochondria together with an increase in the specific surface of cristae .
	manualset3
170609	1	413165	7	NULL	NULL	0	NULL	cross-resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is broad cross-resistance between RAL and EVG , which should preclude their sequential use .
	manualset3
170610	2	413165	7	NULL	NULL	0	NULL	RAL	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	There is broad cross-resistance between RAL and EVG , which should preclude their sequential use .
	manualset3
170611	3	413165	7	NULL	NULL	0	NULL	EVG	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	There is broad cross-resistance between RAL and EVG , which should preclude their sequential use .
	manualset3
170612	4	413165	7	NULL	NULL	0	NULL	sequential use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is broad cross-resistance between RAL and EVG , which should preclude their sequential use .
	manualset3
170613	1	413166	7	NULL	NULL	0	NULL	 debate	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is currently a debate as to whether event-related potentials and fields measured by using electroencephalography or magnetoencephalography are generated by ongoing oscillatory activity becoming phase-reset in response to a given stimulus .
	manualset3
170614	2	413166	7	NULL	NULL	0	NULL	event-related potentials	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There is currently a debate as to whether event-related potentials and fields measured by using electroencephalography or magnetoencephalography are generated by ongoing oscillatory activity becoming phase-reset in response to a given stimulus .
	manualset3
170615	3	413166	7	NULL	NULL	0	NULL	fields	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There is currently a debate as to whether event-related potentials and fields measured by using electroencephalography or magnetoencephalography are generated by ongoing oscillatory activity becoming phase-reset in response to a given stimulus .
	manualset3
170616	4	413166	7	NULL	NULL	0	NULL	electroencephalography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There is currently a debate as to whether event-related potentials and fields measured by using electroencephalography or magnetoencephalography are generated by ongoing oscillatory activity becoming phase-reset in response to a given stimulus .
	manualset3
170617	5	413166	7	NULL	NULL	0	NULL	magnetoencephalography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There is currently a debate as to whether event-related potentials and fields measured by using electroencephalography or magnetoencephalography are generated by ongoing oscillatory activity becoming phase-reset in response to a given stimulus .
	manualset3
170618	6	413166	7	NULL	NULL	0	NULL	ongoing oscillatory activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is currently a debate as to whether event-related potentials and fields measured by using electroencephalography or magnetoencephalography are generated by ongoing oscillatory activity becoming phase-reset in response to a given stimulus .
	manualset3
170619	7	413166	7	NULL	NULL	0	NULL	phase-reset	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is currently a debate as to whether event-related potentials and fields measured by using electroencephalography or magnetoencephalography are generated by ongoing oscillatory activity becoming phase-reset in response to a given stimulus .
	manualset3
170620	8	413166	7	NULL	NULL	0	NULL	 response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There is currently a debate as to whether event-related potentials and fields measured by using electroencephalography or magnetoencephalography are generated by ongoing oscillatory activity becoming phase-reset in response to a given stimulus .
	manualset3
170621	9	413166	7	NULL	NULL	NULL	NULL	stimulus 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There is currently a debate as to whether event-related potentials and fields measured by using electroencephalography or magnetoencephalography are generated by ongoing oscillatory activity becoming phase-reset in response to a given stimulus .
	manualset3
170622	1	413167	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is evidence for a role of insulin and leptin in food intake , but the effects of these adiposity signals on the brain reward system are not well understood .
	manualset3
170623	2	413167	7	NULL	NULL	NULL	NULL	role	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There is evidence for a role of insulin and leptin in food intake , but the effects of these adiposity signals on the brain reward system are not well understood .
	manualset3
170624	3	413167	7	NULL	NULL	0	NULL	insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	There is evidence for a role of insulin and leptin in food intake , but the effects of these adiposity signals on the brain reward system are not well understood .
	manualset3
170625	4	413167	7	NULL	NULL	0	NULL	leptin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	There is evidence for a role of insulin and leptin in food intake , but the effects of these adiposity signals on the brain reward system are not well understood .
	manualset3
170626	5	413167	7	NULL	NULL	0	NULL	 food intake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There is evidence for a role of insulin and leptin in food intake , but the effects of these adiposity signals on the brain reward system are not well understood .
	manualset3
170627	6	413167	7	NULL	NULL	0	NULL	effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There is evidence for a role of insulin and leptin in food intake , but the effects of these adiposity signals on the brain reward system are not well understood .
	manualset3
170628	7	413167	7	NULL	NULL	NULL	NULL	adiposity signals	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There is evidence for a role of insulin and leptin in food intake , but the effects of these adiposity signals on the brain reward system are not well understood .
	manualset3
170629	8	413167	7	NULL	NULL	0	NULL	brain reward system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There is evidence for a role of insulin and leptin in food intake , but the effects of these adiposity signals on the brain reward system are not well understood .
	manualset3
170630	1	413168	7	NULL	NULL	0	NULL	Activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of the p38 Map kinase pathway is essential for the antileukemic effects of dasatinib .
	manualset3
170631	2	413168	7	NULL	NULL	0	NULL	p38 Map kinase pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of the p38 Map kinase pathway is essential for the antileukemic effects of dasatinib .
	manualset3
170632	3	413168	7	NULL	NULL	0	NULL	antileukemic effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of the p38 Map kinase pathway is essential for the antileukemic effects of dasatinib .
	manualset3
170633	4	413168	7	NULL	NULL	0	NULL	dasatinib	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of the p38 Map kinase pathway is essential for the antileukemic effects of dasatinib .
	manualset3
170634	1	413169	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is evidence implying an active role of airway epithelium in the modulation of bronchomotor tone .
	manualset3
170635	2	413169	7	NULL	NULL	0	NULL	active role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There is evidence implying an active role of airway epithelium in the modulation of bronchomotor tone .
	manualset3
170636	3	413169	7	NULL	NULL	0	NULL	airway epithelium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There is evidence implying an active role of airway epithelium in the modulation of bronchomotor tone .
	manualset3
170637	4	413169	7	NULL	NULL	0	NULL	modulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There is evidence implying an active role of airway epithelium in the modulation of bronchomotor tone .
	manualset3
170638	5	413169	7	NULL	NULL	0	NULL	bronchomotor tone	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is evidence implying an active role of airway epithelium in the modulation of bronchomotor tone .
	manualset3
170639	1	413170	7	NULL	NULL	0	NULL	 evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is evidence that reducing the overall times for an oncology care process has a major impact on outcome for patients .
	manualset3
170640	2	413170	7	NULL	NULL	0	NULL	overall times	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	There is evidence that reducing the overall times for an oncology care process has a major impact on outcome for patients .
	manualset3
170641	3	413170	7	NULL	NULL	0	NULL	oncology care process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is evidence that reducing the overall times for an oncology care process has a major impact on outcome for patients .
	manualset3
170642	4	413170	7	NULL	NULL	0	NULL	outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is evidence that reducing the overall times for an oncology care process has a major impact on outcome for patients .
	manualset3
170643	5	413170	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There is evidence that reducing the overall times for an oncology care process has a major impact on outcome for patients .
	manualset3
170644	6	413170	7	NULL	NULL	0	NULL	major impact 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is evidence that reducing the overall times for an oncology care process has a major impact on outcome for patients .
	manualset3
170645	1	413171	7	NULL	NULL	NULL	NULL	extensive junctional contact	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There is extensive junctional contact between the SR and T system .
	manualset3
170646	2	413171	7	NULL	NULL	0	NULL	SR and T system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	There is extensive junctional contact between the SR and T system .
	manualset3
170647	1	413172	7	NULL	NULL	0	NULL	 histological evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is histological evidence the APF proceeded a percutaneous liver biopsy performed 26 years ago .
	manualset3
170648	2	413172	7	NULL	NULL	0	NULL	APF	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is histological evidence the APF proceeded a percutaneous liver biopsy performed 26 years ago .
	manualset3
170649	3	413172	7	NULL	NULL	0	NULL	 percutaneous liver biopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There is histological evidence the APF proceeded a percutaneous liver biopsy performed 26 years ago .
	manualset3
170650	4	413172	7	NULL	NULL	0	NULL	26 years ago	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	There is histological evidence the APF proceeded a percutaneous liver biopsy performed 26 years ago .
	manualset3
170651	1	413173	7	NULL	NULL	0	NULL	increasing evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence that TNF - may play a critical role in skeletal muscle atrophy .
	manualset3
170652	2	413173	7	NULL	NULL	0	NULL	TNF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence that TNF - may play a critical role in skeletal muscle atrophy .
	manualset3
170653	3	413173	7	NULL	NULL	0	NULL	critical role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence that TNF - may play a critical role in skeletal muscle atrophy .
	manualset3
170654	4	413173	7	NULL	NULL	0	NULL	skeletal muscle atrophy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence that TNF - may play a critical role in skeletal muscle atrophy .
	manualset3
170655	1	413174	7	NULL	NULL	0	NULL	 increasing evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence that the reassortment of virulence factor repertoires by converting phages like the GIFSY phages and SopEPhi may represent an important mechanism in the adaptation of Salmonella spp .
	manualset3
170656	2	413174	7	NULL	NULL	0	NULL	 reassortment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence that the reassortment of virulence factor repertoires by converting phages like the GIFSY phages and SopEPhi may represent an important mechanism in the adaptation of Salmonella spp .
	manualset3
170657	3	413174	7	NULL	NULL	0	NULL	virulence factor repertoires	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence that the reassortment of virulence factor repertoires by converting phages like the GIFSY phages and SopEPhi may represent an important mechanism in the adaptation of Salmonella spp .
	manualset3
170658	4	413174	7	NULL	NULL	0	NULL	converting phages	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence that the reassortment of virulence factor repertoires by converting phages like the GIFSY phages and SopEPhi may represent an important mechanism in the adaptation of Salmonella spp .
	manualset3
170659	5	413174	7	NULL	NULL	0	NULL	GIFSY phages	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence that the reassortment of virulence factor repertoires by converting phages like the GIFSY phages and SopEPhi may represent an important mechanism in the adaptation of Salmonella spp .
	manualset3
170660	6	413174	7	NULL	NULL	0	NULL	SopEPhi	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence that the reassortment of virulence factor repertoires by converting phages like the GIFSY phages and SopEPhi may represent an important mechanism in the adaptation of Salmonella spp .
	manualset3
170661	7	413174	7	NULL	NULL	0	NULL	important mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence that the reassortment of virulence factor repertoires by converting phages like the GIFSY phages and SopEPhi may represent an important mechanism in the adaptation of Salmonella spp .
	manualset3
170662	8	413174	7	NULL	NULL	0	NULL	adaptation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence that the reassortment of virulence factor repertoires by converting phages like the GIFSY phages and SopEPhi may represent an important mechanism in the adaptation of Salmonella spp .
	manualset3
170663	9	413174	7	NULL	NULL	0	NULL	Salmonella spp	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence that the reassortment of virulence factor repertoires by converting phages like the GIFSY phages and SopEPhi may represent an important mechanism in the adaptation of Salmonella spp .
	manualset3
170664	1	413175	7	NULL	NULL	0	NULL	 increasing evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence that variation in glucose homeostasis reflects genetic control better than that of commonly used surrogate measures ( fasting glucose or fasting insulin ) .
	manualset3
170665	2	413175	7	NULL	NULL	0	NULL	 variation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence that variation in glucose homeostasis reflects genetic control better than that of commonly used surrogate measures ( fasting glucose or fasting insulin ) .
	manualset3
170666	3	413175	7	NULL	NULL	0	NULL	glucose homeostasis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence that variation in glucose homeostasis reflects genetic control better than that of commonly used surrogate measures ( fasting glucose or fasting insulin ) .
	manualset3
170667	4	413175	7	NULL	NULL	0	NULL	genetic control	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence that variation in glucose homeostasis reflects genetic control better than that of commonly used surrogate measures ( fasting glucose or fasting insulin ) .
	manualset3
170668	5	413175	7	NULL	NULL	0	NULL	 surrogate measures	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence that variation in glucose homeostasis reflects genetic control better than that of commonly used surrogate measures ( fasting glucose or fasting insulin ) .
	manualset3
170669	6	413175	7	NULL	NULL	0	NULL	fasting glucose	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence that variation in glucose homeostasis reflects genetic control better than that of commonly used surrogate measures ( fasting glucose or fasting insulin ) .
	manualset3
170670	7	413175	7	NULL	NULL	0	NULL	fasting insulin	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence that variation in glucose homeostasis reflects genetic control better than that of commonly used surrogate measures ( fasting glucose or fasting insulin ) .
	manualset3
170671	1	413176	7	NULL	NULL	0	NULL	 increasing evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence that vascular risk factors including hypertension , high cholesterol , hyperhomocysteinemia and diabetes mellitus are connected to the risk of Alzheimer 's disease ( AD ) .
	manualset3
170672	2	413176	7	NULL	NULL	0	NULL	vascular risk factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence that vascular risk factors including hypertension , high cholesterol , hyperhomocysteinemia and diabetes mellitus are connected to the risk of Alzheimer 's disease ( AD ) .
	manualset3
170673	3	413176	7	NULL	NULL	0	NULL	hypertension 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence that vascular risk factors including hypertension , high cholesterol , hyperhomocysteinemia and diabetes mellitus are connected to the risk of Alzheimer 's disease ( AD ) .
	manualset3
170674	4	413176	7	NULL	NULL	0	NULL	high cholesterol 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence that vascular risk factors including hypertension , high cholesterol , hyperhomocysteinemia and diabetes mellitus are connected to the risk of Alzheimer 's disease ( AD ) .
	manualset3
170675	5	413176	7	NULL	NULL	0	NULL	hyperhomocysteinemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence that vascular risk factors including hypertension , high cholesterol , hyperhomocysteinemia and diabetes mellitus are connected to the risk of Alzheimer 's disease ( AD ) .
	manualset3
170676	6	413176	7	NULL	NULL	0	NULL	diabetes mellitus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence that vascular risk factors including hypertension , high cholesterol , hyperhomocysteinemia and diabetes mellitus are connected to the risk of Alzheimer 's disease ( AD ) .
	manualset3
170677	7	413176	7	NULL	NULL	0	NULL	 risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence that vascular risk factors including hypertension , high cholesterol , hyperhomocysteinemia and diabetes mellitus are connected to the risk of Alzheimer 's disease ( AD ) .
	manualset3
170678	8	413176	7	NULL	NULL	0	NULL	Alzheimer 's disease ( AD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence that vascular risk factors including hypertension , high cholesterol , hyperhomocysteinemia and diabetes mellitus are connected to the risk of Alzheimer 's disease ( AD ) .
	manualset3
170679	1	413177	7	NULL	NULL	0	NULL	 increasing experimental evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing experimental evidence that oxidation of LDL plays a major role in the pathogenesis of coronary artery disease ( CAD ) .
	manualset3
170680	2	413177	7	NULL	NULL	0	NULL	oxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing experimental evidence that oxidation of LDL plays a major role in the pathogenesis of coronary artery disease ( CAD ) .
	manualset3
170681	3	413177	7	NULL	NULL	0	NULL	LDL	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing experimental evidence that oxidation of LDL plays a major role in the pathogenesis of coronary artery disease ( CAD ) .
	manualset3
170682	4	413177	7	NULL	NULL	NULL	NULL	 role 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There is increasing experimental evidence that oxidation of LDL plays a major role in the pathogenesis of coronary artery disease ( CAD ) .
	manualset3
170683	5	413177	7	NULL	NULL	0	NULL	 pathogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing experimental evidence that oxidation of LDL plays a major role in the pathogenesis of coronary artery disease ( CAD ) .
	manualset3
170684	6	413177	7	NULL	NULL	0	NULL	coronary artery disease ( CAD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing experimental evidence that oxidation of LDL plays a major role in the pathogenesis of coronary artery disease ( CAD ) .
	manualset3
170685	1	413178	7	NULL	NULL	0	NULL	Activation patterns	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation patterns of the four thigh muscles ( rectus femoris , vastus medialis , vastus lateralis and semimembranosus ) were investigated in static leg extension through the entire range of extension movement in three testing postures : sitting , recumbent and supine .
	manualset3
170686	2	413178	7	NULL	NULL	0	NULL	 four thigh muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation patterns of the four thigh muscles ( rectus femoris , vastus medialis , vastus lateralis and semimembranosus ) were investigated in static leg extension through the entire range of extension movement in three testing postures : sitting , recumbent and supine .
	manualset3
170687	3	413178	7	NULL	NULL	0	NULL	 rectus femoris 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation patterns of the four thigh muscles ( rectus femoris , vastus medialis , vastus lateralis and semimembranosus ) were investigated in static leg extension through the entire range of extension movement in three testing postures : sitting , recumbent and supine .
	manualset3
170688	4	413178	7	NULL	NULL	0	NULL	vastus medialis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation patterns of the four thigh muscles ( rectus femoris , vastus medialis , vastus lateralis and semimembranosus ) were investigated in static leg extension through the entire range of extension movement in three testing postures : sitting , recumbent and supine .
	manualset3
170689	5	413178	7	NULL	NULL	0	NULL	vastus lateralis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation patterns of the four thigh muscles ( rectus femoris , vastus medialis , vastus lateralis and semimembranosus ) were investigated in static leg extension through the entire range of extension movement in three testing postures : sitting , recumbent and supine .
	manualset3
170690	6	413178	7	NULL	NULL	0	NULL	semimembranosus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation patterns of the four thigh muscles ( rectus femoris , vastus medialis , vastus lateralis and semimembranosus ) were investigated in static leg extension through the entire range of extension movement in three testing postures : sitting , recumbent and supine .
	manualset3
170691	7	413178	7	NULL	NULL	0	NULL	static leg extension	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation patterns of the four thigh muscles ( rectus femoris , vastus medialis , vastus lateralis and semimembranosus ) were investigated in static leg extension through the entire range of extension movement in three testing postures : sitting , recumbent and supine .
	manualset3
170692	8	413178	7	NULL	NULL	0	NULL	entire range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation patterns of the four thigh muscles ( rectus femoris , vastus medialis , vastus lateralis and semimembranosus ) were investigated in static leg extension through the entire range of extension movement in three testing postures : sitting , recumbent and supine .
	manualset3
170693	9	413178	7	NULL	NULL	0	NULL	extension movement	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation patterns of the four thigh muscles ( rectus femoris , vastus medialis , vastus lateralis and semimembranosus ) were investigated in static leg extension through the entire range of extension movement in three testing postures : sitting , recumbent and supine .
	manualset3
170694	10	413178	7	NULL	NULL	0	NULL	three testing postures	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation patterns of the four thigh muscles ( rectus femoris , vastus medialis , vastus lateralis and semimembranosus ) were investigated in static leg extension through the entire range of extension movement in three testing postures : sitting , recumbent and supine .
	manualset3
170695	11	413178	7	NULL	NULL	0	NULL	 sitting	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation patterns of the four thigh muscles ( rectus femoris , vastus medialis , vastus lateralis and semimembranosus ) were investigated in static leg extension through the entire range of extension movement in three testing postures : sitting , recumbent and supine .
	manualset3
170696	12	413178	7	NULL	NULL	0	NULL	recumbent 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation patterns of the four thigh muscles ( rectus femoris , vastus medialis , vastus lateralis and semimembranosus ) were investigated in static leg extension through the entire range of extension movement in three testing postures : sitting , recumbent and supine .
	manualset3
170697	13	413178	7	NULL	NULL	0	NULL	supine 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation patterns of the four thigh muscles ( rectus femoris , vastus medialis , vastus lateralis and semimembranosus ) were investigated in static leg extension through the entire range of extension movement in three testing postures : sitting , recumbent and supine .
	manualset3
170698	1	413179	7	NULL	NULL	0	NULL	indirect evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is indirect evidence showing that either transient or stable expression of HC-Pro in plants results in an increase of non-methylated small RNAs .
	manualset3
170699	2	413179	7	NULL	NULL	0	NULL	transient expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There is indirect evidence showing that either transient or stable expression of HC-Pro in plants results in an increase of non-methylated small RNAs .
	manualset3
170700	3	413179	7	NULL	NULL	0	NULL	stable expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There is indirect evidence showing that either transient or stable expression of HC-Pro in plants results in an increase of non-methylated small RNAs .
	manualset3
170701	4	413179	7	NULL	NULL	NULL	NULL	HC-Pro	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There is indirect evidence showing that either transient or stable expression of HC-Pro in plants results in an increase of non-methylated small RNAs .
	manualset3
170702	5	413179	7	NULL	NULL	0	NULL	plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	There is indirect evidence showing that either transient or stable expression of HC-Pro in plants results in an increase of non-methylated small RNAs .
	manualset3
170703	6	413179	7	NULL	NULL	0	NULL	increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There is indirect evidence showing that either transient or stable expression of HC-Pro in plants results in an increase of non-methylated small RNAs .
	manualset3
170704	7	413179	7	NULL	NULL	0	NULL	non-methylated small RNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	There is indirect evidence showing that either transient or stable expression of HC-Pro in plants results in an increase of non-methylated small RNAs .
	manualset3
170705	1	413180	7	NULL	NULL	0	NULL	 little information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	There is little information on angiogenesis and no available data on lymphangiogenesis in parathyroid glands ( PTG ) .
	manualset3
170706	2	413180	7	NULL	NULL	0	NULL	angiogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There is little information on angiogenesis and no available data on lymphangiogenesis in parathyroid glands ( PTG ) .
	manualset3
170707	3	413180	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	There is little information on angiogenesis and no available data on lymphangiogenesis in parathyroid glands ( PTG ) .
	manualset3
170708	4	413180	7	NULL	NULL	0	NULL	lymphangiogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There is little information on angiogenesis and no available data on lymphangiogenesis in parathyroid glands ( PTG ) .
	manualset3
170709	5	413180	7	NULL	NULL	0	NULL	parathyroid glands ( PTG )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There is little information on angiogenesis and no available data on lymphangiogenesis in parathyroid glands ( PTG ) .
	manualset3
170710	1	413181	7	NULL	NULL	0	NULL	question	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is little question among members of the profession that practitioners are faced with crucial survival issues in this decade and the next .
	manualset3
170711	2	413181	7	NULL	NULL	0	NULL	members	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There is little question among members of the profession that practitioners are faced with crucial survival issues in this decade and the next .
	manualset3
170712	3	413181	7	NULL	NULL	0	NULL	profession	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There is little question among members of the profession that practitioners are faced with crucial survival issues in this decade and the next .
	manualset3
170713	4	413181	7	NULL	NULL	0	NULL	practitioners	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There is little question among members of the profession that practitioners are faced with crucial survival issues in this decade and the next .
	manualset3
170714	5	413181	7	NULL	NULL	0	NULL	crucial survival issues	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is little question among members of the profession that practitioners are faced with crucial survival issues in this decade and the next .
	manualset3
170715	6	413181	7	NULL	NULL	0	NULL	 decade	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	There is little question among members of the profession that practitioners are faced with crucial survival issues in this decade and the next .
	manualset3
170716	1	413182	7	NULL	NULL	0	NULL	minimal potentiation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is minimal potentiation for QTC prolongation , and they are safe and effective as first-line therapies for seasonal allergic rhinitis .
	manualset3
170717	2	413182	7	NULL	NULL	0	NULL	 QTC prolongation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is minimal potentiation for QTC prolongation , and they are safe and effective as first-line therapies for seasonal allergic rhinitis .
	manualset3
170719	4	413182	7	NULL	NULL	0	NULL	first-line therapies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There is minimal potentiation for QTC prolongation , and they are safe and effective as first-line therapies for seasonal allergic rhinitis .
	manualset3
170720	5	413182	7	NULL	NULL	0	NULL	seasonal allergic rhinitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is minimal potentiation for QTC prolongation , and they are safe and effective as first-line therapies for seasonal allergic rhinitis .
	manualset3
170721	1	413183	7	NULL	NULL	NULL	NULL	evidence of benefit	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There is neither evidence of benefit in withholding fluids nor evidence of risk in allowing them .
	manualset3
170722	2	413183	7	NULL	NULL	0	NULL	withholding fluids	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is neither evidence of benefit in withholding fluids nor evidence of risk in allowing them .
	manualset3
170723	3	413183	7	NULL	NULL	0	NULL	 evidence of risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is neither evidence of benefit in withholding fluids nor evidence of risk in allowing them .
	manualset3
170724	1	413184	7	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There is no apparent correlation between conformational properties and the nature of the Xaa side chain within the two groups .
	manualset3
170725	2	413184	7	NULL	NULL	0	NULL	conformational properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There is no apparent correlation between conformational properties and the nature of the Xaa side chain within the two groups .
	manualset3
170726	3	413184	7	NULL	NULL	0	NULL	nature	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is no apparent correlation between conformational properties and the nature of the Xaa side chain within the two groups .
	manualset3
170727	4	413184	7	NULL	NULL	0	NULL	Xaa side chain	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There is no apparent correlation between conformational properties and the nature of the Xaa side chain within the two groups .
	manualset3
170728	5	413184	7	NULL	NULL	0	NULL	two groups 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There is no apparent correlation between conformational properties and the nature of the Xaa side chain within the two groups .
	manualset3
170729	1	413185	7	NULL	NULL	0	NULL	Active-site inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Active and exo-site inhibition of human factor Xa : structure of des-Gla factor Xa inhibited by NAP5 , a potent nematode anticoagulant protein from Ancylostoma caninum .
	manualset3
170730	2	413185	7	NULL	NULL	0	NULL	exo-site inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Active and exo-site inhibition of human factor Xa : structure of des-Gla factor Xa inhibited by NAP5 , a potent nematode anticoagulant protein from Ancylostoma caninum .
	manualset3
170731	3	413185	7	NULL	NULL	0	NULL	human factor Xa	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Active and exo-site inhibition of human factor Xa : structure of des-Gla factor Xa inhibited by NAP5 , a potent nematode anticoagulant protein from Ancylostoma caninum .
	manualset3
170732	4	413185	7	NULL	NULL	0	NULL	structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Active and exo-site inhibition of human factor Xa : structure of des-Gla factor Xa inhibited by NAP5 , a potent nematode anticoagulant protein from Ancylostoma caninum .
	manualset3
170733	5	413185	7	NULL	NULL	0	NULL	des-Gla factor Xa	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Active and exo-site inhibition of human factor Xa : structure of des-Gla factor Xa inhibited by NAP5 , a potent nematode anticoagulant protein from Ancylostoma caninum .
	manualset3
170734	6	413185	7	NULL	NULL	0	NULL	NAP5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Active and exo-site inhibition of human factor Xa : structure of des-Gla factor Xa inhibited by NAP5 , a potent nematode anticoagulant protein from Ancylostoma caninum .
	manualset3
170735	7	413185	7	NULL	NULL	0	NULL	nematode anticoagulant protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Active and exo-site inhibition of human factor Xa : structure of des-Gla factor Xa inhibited by NAP5 , a potent nematode anticoagulant protein from Ancylostoma caninum .
	manualset3
170736	8	413185	7	NULL	NULL	0	NULL	Ancylostoma caninum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Active and exo-site inhibition of human factor Xa : structure of des-Gla factor Xa inhibited by NAP5 , a potent nematode anticoagulant protein from Ancylostoma caninum .
	manualset3
170737	1	413186	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is now evidence that the actions of chemotherapy may involve Ras , tyrosine kinases ( epidermal growth factor receptor , HER2 ) , TC21 , or similar molecules .
	manualset3
170738	2	413186	7	NULL	NULL	0	NULL	actions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There is now evidence that the actions of chemotherapy may involve Ras , tyrosine kinases ( epidermal growth factor receptor , HER2 ) , TC21 , or similar molecules .
	manualset3
170739	3	413186	7	NULL	NULL	0	NULL	chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There is now evidence that the actions of chemotherapy may involve Ras , tyrosine kinases ( epidermal growth factor receptor , HER2 ) , TC21 , or similar molecules .
	manualset3
170740	4	413186	7	NULL	NULL	0	NULL	Ras	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	There is now evidence that the actions of chemotherapy may involve Ras , tyrosine kinases ( epidermal growth factor receptor , HER2 ) , TC21 , or similar molecules .
	manualset3
170741	5	413186	7	NULL	NULL	0	NULL	 tyrosine kinases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There is now evidence that the actions of chemotherapy may involve Ras , tyrosine kinases ( epidermal growth factor receptor , HER2 ) , TC21 , or similar molecules .
	manualset3
170742	6	413186	7	NULL	NULL	0	NULL	epidermal growth factor receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	There is now evidence that the actions of chemotherapy may involve Ras , tyrosine kinases ( epidermal growth factor receptor , HER2 ) , TC21 , or similar molecules .
	manualset3
170743	7	413186	7	NULL	NULL	0	NULL	HER2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	There is now evidence that the actions of chemotherapy may involve Ras , tyrosine kinases ( epidermal growth factor receptor , HER2 ) , TC21 , or similar molecules .
	manualset3
170744	8	413186	7	NULL	NULL	0	NULL	TC21	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	There is now evidence that the actions of chemotherapy may involve Ras , tyrosine kinases ( epidermal growth factor receptor , HER2 ) , TC21 , or similar molecules .
	manualset3
170745	9	413186	7	NULL	NULL	0	NULL	molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	There is now evidence that the actions of chemotherapy may involve Ras , tyrosine kinases ( epidermal growth factor receptor , HER2 ) , TC21 , or similar molecules .
	manualset3
170746	1	413187	7	NULL	NULL	0	NULL	world-wide concern	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is now world-wide concern for the quantification of lung cancer risk due to indoor radon , but the recent estimates are based on epidemiological studies of miners alone .
	manualset3
170747	2	413187	7	NULL	NULL	0	NULL	quantification	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There is now world-wide concern for the quantification of lung cancer risk due to indoor radon , but the recent estimates are based on epidemiological studies of miners alone .
	manualset3
170748	3	413187	7	NULL	NULL	0	NULL	lung cancer risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is now world-wide concern for the quantification of lung cancer risk due to indoor radon , but the recent estimates are based on epidemiological studies of miners alone .
	manualset3
170749	4	413187	7	NULL	NULL	0	NULL	 indoor radon 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There is now world-wide concern for the quantification of lung cancer risk due to indoor radon , but the recent estimates are based on epidemiological studies of miners alone .
	manualset3
170750	5	413187	7	NULL	NULL	0	NULL	 estimates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There is now world-wide concern for the quantification of lung cancer risk due to indoor radon , but the recent estimates are based on epidemiological studies of miners alone .
	manualset3
170751	6	413187	7	NULL	NULL	0	NULL	epidemiological studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	There is now world-wide concern for the quantification of lung cancer risk due to indoor radon , but the recent estimates are based on epidemiological studies of miners alone .
	manualset3
170752	7	413187	7	NULL	NULL	0	NULL	miners	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There is now world-wide concern for the quantification of lung cancer risk due to indoor radon , but the recent estimates are based on epidemiological studies of miners alone .
	manualset3
170753	1	413188	7	NULL	NULL	0	NULL	 evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is strong evidence which suggests that synergistic binding of hydrophobic residues drives binding of OVIS to the micelle .
	manualset3
170754	2	413188	7	NULL	NULL	0	NULL	synergistic binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There is strong evidence which suggests that synergistic binding of hydrophobic residues drives binding of OVIS to the micelle .
	manualset3
170755	3	413188	7	NULL	NULL	0	NULL	hydrophobic residues 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There is strong evidence which suggests that synergistic binding of hydrophobic residues drives binding of OVIS to the micelle .
	manualset3
170756	4	413188	7	NULL	NULL	0	NULL	 binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There is strong evidence which suggests that synergistic binding of hydrophobic residues drives binding of OVIS to the micelle .
	manualset3
170757	5	413188	7	NULL	NULL	0	NULL	OVIS	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	There is strong evidence which suggests that synergistic binding of hydrophobic residues drives binding of OVIS to the micelle .
	manualset3
170758	6	413188	7	NULL	NULL	0	NULL	micelle	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There is strong evidence which suggests that synergistic binding of hydrophobic residues drives binding of OVIS to the micelle .
	manualset3
170759	1	413189	7	NULL	NULL	0	NULL	need	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is therefore , need to improve sewage and refuse disposal system , the provision of safe potable water , sanitation , personal hygiene and health education in order to reduce infection with this and other enteric pathogens .
	manualset3
170760	2	413189	7	NULL	NULL	0	NULL	 sewage disposal system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	There is therefore , need to improve sewage and refuse disposal system , the provision of safe potable water , sanitation , personal hygiene and health education in order to reduce infection with this and other enteric pathogens .
	manualset3
170761	3	413189	7	NULL	NULL	0	NULL	refuse disposal system 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	There is therefore , need to improve sewage and refuse disposal system , the provision of safe potable water , sanitation , personal hygiene and health education in order to reduce infection with this and other enteric pathogens .
	manualset3
170762	4	413189	7	NULL	NULL	0	NULL	provision	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is therefore , need to improve sewage and refuse disposal system , the provision of safe potable water , sanitation , personal hygiene and health education in order to reduce infection with this and other enteric pathogens .
	manualset3
170763	5	413189	7	NULL	NULL	0	NULL	safe potable water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There is therefore , need to improve sewage and refuse disposal system , the provision of safe potable water , sanitation , personal hygiene and health education in order to reduce infection with this and other enteric pathogens .
	manualset3
170764	6	413189	7	NULL	NULL	0	NULL	sanitation	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	There is therefore , need to improve sewage and refuse disposal system , the provision of safe potable water , sanitation , personal hygiene and health education in order to reduce infection with this and other enteric pathogens .
	manualset3
170765	7	413189	7	NULL	NULL	0	NULL	personal hygiene	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is therefore , need to improve sewage and refuse disposal system , the provision of safe potable water , sanitation , personal hygiene and health education in order to reduce infection with this and other enteric pathogens .
	manualset3
170766	8	413189	7	NULL	NULL	0	NULL	health education	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	There is therefore , need to improve sewage and refuse disposal system , the provision of safe potable water , sanitation , personal hygiene and health education in order to reduce infection with this and other enteric pathogens .
	manualset3
170767	9	413189	7	NULL	NULL	0	NULL	 infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is therefore , need to improve sewage and refuse disposal system , the provision of safe potable water , sanitation , personal hygiene and health education in order to reduce infection with this and other enteric pathogens .
	manualset3
170768	10	413189	7	NULL	NULL	0	NULL	enteric pathogens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	There is therefore , need to improve sewage and refuse disposal system , the provision of safe potable water , sanitation , personal hygiene and health education in order to reduce infection with this and other enteric pathogens .
	manualset3
170769	1	413190	7	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a clear correlation between the percentage of blast cells and the enzyme activity when mononuclear cell fractions from patient samples were analyzed .
	manualset3
170770	2	413190	7	NULL	NULL	0	NULL	 percentage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a clear correlation between the percentage of blast cells and the enzyme activity when mononuclear cell fractions from patient samples were analyzed .
	manualset3
170771	3	413190	7	NULL	NULL	0	NULL	blast cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a clear correlation between the percentage of blast cells and the enzyme activity when mononuclear cell fractions from patient samples were analyzed .
	manualset3
170772	4	413190	7	NULL	NULL	0	NULL	enzyme activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a clear correlation between the percentage of blast cells and the enzyme activity when mononuclear cell fractions from patient samples were analyzed .
	manualset3
170773	5	413190	7	NULL	NULL	0	NULL	mononuclear cell fractions	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a clear correlation between the percentage of blast cells and the enzyme activity when mononuclear cell fractions from patient samples were analyzed .
	manualset3
170774	6	413190	7	NULL	NULL	0	NULL	patient samples	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a clear correlation between the percentage of blast cells and the enzyme activity when mononuclear cell fractions from patient samples were analyzed .
	manualset3
170775	1	413191	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a clear relationship with the aggressiveness of therapy , because 81.7 % of the viral episodes occurred in patients submitted to total radiotherapy with or without chemotherapy , or with partial radiotherapy plus chemotherapy .
	manualset3
170776	2	413191	7	NULL	NULL	0	NULL	aggressiveness	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a clear relationship with the aggressiveness of therapy , because 81.7 % of the viral episodes occurred in patients submitted to total radiotherapy with or without chemotherapy , or with partial radiotherapy plus chemotherapy .
	manualset3
170777	3	413191	7	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a clear relationship with the aggressiveness of therapy , because 81.7 % of the viral episodes occurred in patients submitted to total radiotherapy with or without chemotherapy , or with partial radiotherapy plus chemotherapy .
	manualset3
170778	4	413191	7	NULL	NULL	0	NULL	81.7 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a clear relationship with the aggressiveness of therapy , because 81.7 % of the viral episodes occurred in patients submitted to total radiotherapy with or without chemotherapy , or with partial radiotherapy plus chemotherapy .
	manualset3
170779	5	413191	7	NULL	NULL	0	NULL	viral episodes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a clear relationship with the aggressiveness of therapy , because 81.7 % of the viral episodes occurred in patients submitted to total radiotherapy with or without chemotherapy , or with partial radiotherapy plus chemotherapy .
	manualset3
170780	6	413191	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a clear relationship with the aggressiveness of therapy , because 81.7 % of the viral episodes occurred in patients submitted to total radiotherapy with or without chemotherapy , or with partial radiotherapy plus chemotherapy .
	manualset3
170781	7	413191	7	NULL	NULL	0	NULL	total radiotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a clear relationship with the aggressiveness of therapy , because 81.7 % of the viral episodes occurred in patients submitted to total radiotherapy with or without chemotherapy , or with partial radiotherapy plus chemotherapy .
	manualset3
170782	8	413191	7	NULL	NULL	0	NULL	chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a clear relationship with the aggressiveness of therapy , because 81.7 % of the viral episodes occurred in patients submitted to total radiotherapy with or without chemotherapy , or with partial radiotherapy plus chemotherapy .
	manualset3
170783	9	413191	7	NULL	NULL	0	NULL	partial radiotherapy plus chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a clear relationship with the aggressiveness of therapy , because 81.7 % of the viral episodes occurred in patients submitted to total radiotherapy with or without chemotherapy , or with partial radiotherapy plus chemotherapy .
	manualset3
170784	1	413192	7	NULL	NULL	0	NULL	 relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a close relationship of the number of transfusions of blood plasma to the presence of HCV specific antibody , but not to the serum markers of HBV infection .
	manualset3
170785	2	413192	7	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a close relationship of the number of transfusions of blood plasma to the presence of HCV specific antibody , but not to the serum markers of HBV infection .
	manualset3
170786	3	413192	7	NULL	NULL	0	NULL	transfusions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a close relationship of the number of transfusions of blood plasma to the presence of HCV specific antibody , but not to the serum markers of HBV infection .
	manualset3
170787	4	413192	7	NULL	NULL	0	NULL	blood plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a close relationship of the number of transfusions of blood plasma to the presence of HCV specific antibody , but not to the serum markers of HBV infection .
	manualset3
170788	5	413192	7	NULL	NULL	0	NULL	 presence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a close relationship of the number of transfusions of blood plasma to the presence of HCV specific antibody , but not to the serum markers of HBV infection .
	manualset3
170789	6	413192	7	NULL	NULL	0	NULL	HCV specific antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a close relationship of the number of transfusions of blood plasma to the presence of HCV specific antibody , but not to the serum markers of HBV infection .
	manualset3
170790	7	413192	7	NULL	NULL	0	NULL	serum markers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a close relationship of the number of transfusions of blood plasma to the presence of HCV specific antibody , but not to the serum markers of HBV infection .
	manualset3
170791	8	413192	7	NULL	NULL	0	NULL	HBV infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a close relationship of the number of transfusions of blood plasma to the presence of HCV specific antibody , but not to the serum markers of HBV infection .
	manualset3
170792	1	413193	7	NULL	NULL	0	NULL	 correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a correlation between the ergosterol content of the cell and sensitivity to nystatin , as monitored by both potassium leakage from the cell and viability .
	manualset3
170793	2	413193	7	NULL	NULL	0	NULL	 ergosterol content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a correlation between the ergosterol content of the cell and sensitivity to nystatin , as monitored by both potassium leakage from the cell and viability .
	manualset3
170794	3	413193	7	NULL	NULL	0	NULL	cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a correlation between the ergosterol content of the cell and sensitivity to nystatin , as monitored by both potassium leakage from the cell and viability .
	manualset3
170795	4	413193	7	NULL	NULL	0	NULL	sensitivity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a correlation between the ergosterol content of the cell and sensitivity to nystatin , as monitored by both potassium leakage from the cell and viability .
	manualset3
170796	5	413193	7	NULL	NULL	0	NULL	nystatin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a correlation between the ergosterol content of the cell and sensitivity to nystatin , as monitored by both potassium leakage from the cell and viability .
	manualset3
170797	6	413193	7	NULL	NULL	0	NULL	potassium leakage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a correlation between the ergosterol content of the cell and sensitivity to nystatin , as monitored by both potassium leakage from the cell and viability .
	manualset3
170798	7	413193	7	NULL	NULL	0	NULL	cell 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a correlation between the ergosterol content of the cell and sensitivity to nystatin , as monitored by both potassium leakage from the cell and viability .
	manualset3
170799	8	413193	7	NULL	NULL	NULL	NULL	 viability	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There was a correlation between the ergosterol content of the cell and sensitivity to nystatin , as monitored by both potassium leakage from the cell and viability .
	manualset3
170800	1	413194	7	NULL	NULL	0	NULL	 high rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a high rate of overweight in both males ( 38.7 % ) and females ( 23.5 % ) , and one female adolescent was obese ( 2.9 % ) .
	manualset3
170801	2	413194	7	NULL	NULL	0	NULL	overweight	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a high rate of overweight in both males ( 38.7 % ) and females ( 23.5 % ) , and one female adolescent was obese ( 2.9 % ) .
	manualset3
170802	3	413194	7	NULL	NULL	0	NULL	males	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a high rate of overweight in both males ( 38.7 % ) and females ( 23.5 % ) , and one female adolescent was obese ( 2.9 % ) .
	manualset3
170803	4	413194	7	NULL	NULL	0	NULL	 38.7 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a high rate of overweight in both males ( 38.7 % ) and females ( 23.5 % ) , and one female adolescent was obese ( 2.9 % ) .
	manualset3
170804	5	413194	7	NULL	NULL	0	NULL	females	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a high rate of overweight in both males ( 38.7 % ) and females ( 23.5 % ) , and one female adolescent was obese ( 2.9 % ) .
	manualset3
170805	6	413194	7	NULL	NULL	0	NULL	23.5 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a high rate of overweight in both males ( 38.7 % ) and females ( 23.5 % ) , and one female adolescent was obese ( 2.9 % ) .
	manualset3
170806	7	413194	7	NULL	NULL	0	NULL	one female adolescent	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a high rate of overweight in both males ( 38.7 % ) and females ( 23.5 % ) , and one female adolescent was obese ( 2.9 % ) .
	manualset3
170807	8	413194	7	NULL	NULL	0	NULL	2.9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a high rate of overweight in both males ( 38.7 % ) and females ( 23.5 % ) , and one female adolescent was obese ( 2.9 % ) .
	manualset3
170808	1	413195	7	NULL	NULL	0	NULL	higher degree	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a higher degree of amyloid deposition , overexpression of oxidative stress markers , mitochondria DNA deletion and mitochondrial structural abnormality in the vascular walls of the human AD , YAC and C57B6/SJL Tg ( + ) mice compared to age-matched controls .
	manualset3
170809	2	413195	7	NULL	NULL	0	NULL	amyloid deposition	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a higher degree of amyloid deposition , overexpression of oxidative stress markers , mitochondria DNA deletion and mitochondrial structural abnormality in the vascular walls of the human AD , YAC and C57B6/SJL Tg ( + ) mice compared to age-matched controls .
	manualset3
170810	3	413195	7	NULL	NULL	0	NULL	overexpression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a higher degree of amyloid deposition , overexpression of oxidative stress markers , mitochondria DNA deletion and mitochondrial structural abnormality in the vascular walls of the human AD , YAC and C57B6/SJL Tg ( + ) mice compared to age-matched controls .
	manualset3
170811	4	413195	7	NULL	NULL	0	NULL	oxidative stress markers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a higher degree of amyloid deposition , overexpression of oxidative stress markers , mitochondria DNA deletion and mitochondrial structural abnormality in the vascular walls of the human AD , YAC and C57B6/SJL Tg ( + ) mice compared to age-matched controls .
	manualset3
170812	5	413195	7	NULL	NULL	0	NULL	mitochondria DNA deletion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a higher degree of amyloid deposition , overexpression of oxidative stress markers , mitochondria DNA deletion and mitochondrial structural abnormality in the vascular walls of the human AD , YAC and C57B6/SJL Tg ( + ) mice compared to age-matched controls .
	manualset3
170813	6	413195	7	NULL	NULL	NULL	NULL	mitochondrial structural abnormality	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There was a higher degree of amyloid deposition , overexpression of oxidative stress markers , mitochondria DNA deletion and mitochondrial structural abnormality in the vascular walls of the human AD , YAC and C57B6/SJL Tg ( + ) mice compared to age-matched controls .
	manualset3
170814	7	413195	7	NULL	NULL	0	NULL	vascular walls	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a higher degree of amyloid deposition , overexpression of oxidative stress markers , mitochondria DNA deletion and mitochondrial structural abnormality in the vascular walls of the human AD , YAC and C57B6/SJL Tg ( + ) mice compared to age-matched controls .
	manualset3
170815	8	413195	7	NULL	NULL	0	NULL	human AD	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a higher degree of amyloid deposition , overexpression of oxidative stress markers , mitochondria DNA deletion and mitochondrial structural abnormality in the vascular walls of the human AD , YAC and C57B6/SJL Tg ( + ) mice compared to age-matched controls .
	manualset3
170816	9	413195	7	NULL	NULL	0	NULL	 YAC	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a higher degree of amyloid deposition , overexpression of oxidative stress markers , mitochondria DNA deletion and mitochondrial structural abnormality in the vascular walls of the human AD , YAC and C57B6/SJL Tg ( + ) mice compared to age-matched controls .
	manualset3
170817	10	413195	7	NULL	NULL	0	NULL	 C57B6/SJL Tg ( + ) mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a higher degree of amyloid deposition , overexpression of oxidative stress markers , mitochondria DNA deletion and mitochondrial structural abnormality in the vascular walls of the human AD , YAC and C57B6/SJL Tg ( + ) mice compared to age-matched controls .
	manualset3
170818	11	413195	7	NULL	NULL	0	NULL	age-matched controls	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a higher degree of amyloid deposition , overexpression of oxidative stress markers , mitochondria DNA deletion and mitochondrial structural abnormality in the vascular walls of the human AD , YAC and C57B6/SJL Tg ( + ) mice compared to age-matched controls .
	manualset3
170819	1	413196	7	NULL	NULL	0	NULL	kinetic increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a kinetic increase in the expression of neutrophil C3b receptors in EIA ( + ) asthmatics for up to 60 min after treadmill exercise .
	manualset3
170820	2	413196	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a kinetic increase in the expression of neutrophil C3b receptors in EIA ( + ) asthmatics for up to 60 min after treadmill exercise .
	manualset3
170821	3	413196	7	NULL	NULL	0	NULL	neutrophil C3b receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a kinetic increase in the expression of neutrophil C3b receptors in EIA ( + ) asthmatics for up to 60 min after treadmill exercise .
	manualset3
170822	4	413196	7	NULL	NULL	0	NULL	EIA ( + ) asthmatics	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a kinetic increase in the expression of neutrophil C3b receptors in EIA ( + ) asthmatics for up to 60 min after treadmill exercise .
	manualset3
170823	5	413196	7	NULL	NULL	0	NULL	 60 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a kinetic increase in the expression of neutrophil C3b receptors in EIA ( + ) asthmatics for up to 60 min after treadmill exercise .
	manualset3
170824	6	413196	7	NULL	NULL	0	NULL	 treadmill exercise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a kinetic increase in the expression of neutrophil C3b receptors in EIA ( + ) asthmatics for up to 60 min after treadmill exercise .
	manualset3
170825	1	413197	7	NULL	NULL	0	NULL	 linear correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a linear correlation between PtcCO2 and PaCO2 ( n = 51 , r = .71 , slope = 0.90 ) .
	manualset3
170826	2	413197	7	NULL	NULL	0	NULL	PtcCO2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a linear correlation between PtcCO2 and PaCO2 ( n = 51 , r = .71 , slope = 0.90 ) .
	manualset3
170827	3	413197	7	NULL	NULL	0	NULL	PaCO2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a linear correlation between PtcCO2 and PaCO2 ( n = 51 , r = .71 , slope = 0.90 ) .
	manualset3
170828	4	413197	7	NULL	NULL	0	NULL	 n = 51 , r = .71 , slope = 0.90	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a linear correlation between PtcCO2 and PaCO2 ( n = 51 , r = .71 , slope = 0.90 ) .
	manualset3
170829	1	413198	7	NULL	NULL	NULL	NULL	DNA	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There was a marked decreased in the content of DNA in all three brain regions after the administration of 6 hourly doses of ammonium acetate .
	manualset3
170830	2	413198	7	NULL	NULL	0	NULL	three brain regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a marked decreased in the content of DNA in all three brain regions after the administration of 6 hourly doses of ammonium acetate .
	manualset3
170831	3	413198	7	NULL	NULL	0	NULL	administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a marked decreased in the content of DNA in all three brain regions after the administration of 6 hourly doses of ammonium acetate .
	manualset3
170832	4	413198	7	NULL	NULL	0	NULL	6 hourly doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a marked decreased in the content of DNA in all three brain regions after the administration of 6 hourly doses of ammonium acetate .
	manualset3
170833	5	413198	7	NULL	NULL	0	NULL	ammonium acetate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a marked decreased in the content of DNA in all three brain regions after the administration of 6 hourly doses of ammonium acetate .
	manualset3
170834	6	413198	7	NULL	NULL	0	NULL	content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a marked decreased in the content of DNA in all three brain regions after the administration of 6 hourly doses of ammonium acetate .
	manualset3
170835	1	413199	7	NULL	NULL	0	NULL	Active hypothalamic AMP-activated protein kinase ( AMPK ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Active hypothalamic AMP-activated protein kinase ( AMPK ) has recently been reported to enhance food intake , and in vivo experiments suggested that intrahypothalamic injection of melanocortins decreased food intake due to the inhibition of AMPK activity .
	manualset3
170836	2	413199	7	NULL	NULL	0	NULL	 food intake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Active hypothalamic AMP-activated protein kinase ( AMPK ) has recently been reported to enhance food intake , and in vivo experiments suggested that intrahypothalamic injection of melanocortins decreased food intake due to the inhibition of AMPK activity .
	manualset3
170837	3	413199	7	NULL	NULL	0	NULL	in vivo experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Active hypothalamic AMP-activated protein kinase ( AMPK ) has recently been reported to enhance food intake , and in vivo experiments suggested that intrahypothalamic injection of melanocortins decreased food intake due to the inhibition of AMPK activity .
	manualset3
170838	4	413199	7	NULL	NULL	0	NULL	intrahypothalamic injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Active hypothalamic AMP-activated protein kinase ( AMPK ) has recently been reported to enhance food intake , and in vivo experiments suggested that intrahypothalamic injection of melanocortins decreased food intake due to the inhibition of AMPK activity .
	manualset3
170839	5	413199	7	NULL	NULL	0	NULL	melanocortins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Active hypothalamic AMP-activated protein kinase ( AMPK ) has recently been reported to enhance food intake , and in vivo experiments suggested that intrahypothalamic injection of melanocortins decreased food intake due to the inhibition of AMPK activity .
	manualset3
170840	6	413199	7	NULL	NULL	0	NULL	food intake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Active hypothalamic AMP-activated protein kinase ( AMPK ) has recently been reported to enhance food intake , and in vivo experiments suggested that intrahypothalamic injection of melanocortins decreased food intake due to the inhibition of AMPK activity .
	manualset3
170841	7	413199	7	NULL	NULL	0	NULL	 inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Active hypothalamic AMP-activated protein kinase ( AMPK ) has recently been reported to enhance food intake , and in vivo experiments suggested that intrahypothalamic injection of melanocortins decreased food intake due to the inhibition of AMPK activity .
	manualset3
170842	8	413199	7	NULL	NULL	0	NULL	AMPK activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Active hypothalamic AMP-activated protein kinase ( AMPK ) has recently been reported to enhance food intake , and in vivo experiments suggested that intrahypothalamic injection of melanocortins decreased food intake due to the inhibition of AMPK activity .
	manualset3
170843	1	413200	7	NULL	NULL	NULL	NULL	two-fold interindividual variation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There was a more than two-fold interindividual variation in the plasma concentration during infusion of the standardized doses of phenylephrine , with overlap of the concentrations achieved at the different dose levels .
	manualset3
170844	2	413200	7	NULL	NULL	0	NULL	plasma concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a more than two-fold interindividual variation in the plasma concentration during infusion of the standardized doses of phenylephrine , with overlap of the concentrations achieved at the different dose levels .
	manualset3
170845	3	413200	7	NULL	NULL	0	NULL	infusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a more than two-fold interindividual variation in the plasma concentration during infusion of the standardized doses of phenylephrine , with overlap of the concentrations achieved at the different dose levels .
	manualset3
170846	4	413200	7	NULL	NULL	0	NULL	standardized doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a more than two-fold interindividual variation in the plasma concentration during infusion of the standardized doses of phenylephrine , with overlap of the concentrations achieved at the different dose levels .
	manualset3
170847	5	413200	7	NULL	NULL	0	NULL	phenylephrine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a more than two-fold interindividual variation in the plasma concentration during infusion of the standardized doses of phenylephrine , with overlap of the concentrations achieved at the different dose levels .
	manualset3
170848	6	413200	7	NULL	NULL	0	NULL	overlap	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a more than two-fold interindividual variation in the plasma concentration during infusion of the standardized doses of phenylephrine , with overlap of the concentrations achieved at the different dose levels .
	manualset3
170849	7	413200	7	NULL	NULL	0	NULL	concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a more than two-fold interindividual variation in the plasma concentration during infusion of the standardized doses of phenylephrine , with overlap of the concentrations achieved at the different dose levels .
	manualset3
170850	8	413200	7	NULL	NULL	0	NULL	different dose levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a more than two-fold interindividual variation in the plasma concentration during infusion of the standardized doses of phenylephrine , with overlap of the concentrations achieved at the different dose levels .
	manualset3
170851	1	413201	7	NULL	NULL	0	NULL	positive correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a positive correlation between urinary TGF-beta 1 and plasma glucose levels ( r = 0.65 , p & lt ; 0.05 ) and albuminuria ( r = 0.72 , p & lt ; 0.05 ) .
	manualset3
170852	2	413201	7	NULL	NULL	0	NULL	urinary TGF-beta 1 levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a positive correlation between urinary TGF-beta 1 and plasma glucose levels ( r = 0.65 , p & lt ; 0.05 ) and albuminuria ( r = 0.72 , p & lt ; 0.05 ) .
	manualset3
170853	3	413201	7	NULL	NULL	0	NULL	plasma glucose levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a positive correlation between urinary TGF-beta 1 and plasma glucose levels ( r = 0.65 , p & lt ; 0.05 ) and albuminuria ( r = 0.72 , p & lt ; 0.05 ) .
	manualset3
170854	4	413201	7	NULL	NULL	0	NULL	r = 0.65 , p & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a positive correlation between urinary TGF-beta 1 and plasma glucose levels ( r = 0.65 , p & lt ; 0.05 ) and albuminuria ( r = 0.72 , p & lt ; 0.05 ) .
	manualset3
170855	5	413201	7	NULL	NULL	0	NULL	albuminuria	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a positive correlation between urinary TGF-beta 1 and plasma glucose levels ( r = 0.65 , p & lt ; 0.05 ) and albuminuria ( r = 0.72 , p & lt ; 0.05 ) .
	manualset3
170856	6	413201	7	NULL	NULL	0	NULL	 r = 0.72 , p & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a positive correlation between urinary TGF-beta 1 and plasma glucose levels ( r = 0.65 , p & lt ; 0.05 ) and albuminuria ( r = 0.72 , p & lt ; 0.05 ) .
	manualset3
170857	1	413202	7	NULL	NULL	0	NULL	 positive effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a positive effect of selenium supplementation of the maternal diet on glutathione concentration in the liver of 1-d-old and 5-d-old chicks .
	manualset3
170858	2	413202	7	NULL	NULL	0	NULL	selenium supplementation	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a positive effect of selenium supplementation of the maternal diet on glutathione concentration in the liver of 1-d-old and 5-d-old chicks .
	manualset3
170859	3	413202	7	NULL	NULL	0	NULL	maternal diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a positive effect of selenium supplementation of the maternal diet on glutathione concentration in the liver of 1-d-old and 5-d-old chicks .
	manualset3
170860	4	413202	7	NULL	NULL	0	NULL	glutathione concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a positive effect of selenium supplementation of the maternal diet on glutathione concentration in the liver of 1-d-old and 5-d-old chicks .
	manualset3
170861	5	413202	7	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a positive effect of selenium supplementation of the maternal diet on glutathione concentration in the liver of 1-d-old and 5-d-old chicks .
	manualset3
170862	6	413202	7	NULL	NULL	0	NULL	1-d-old chicks	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a positive effect of selenium supplementation of the maternal diet on glutathione concentration in the liver of 1-d-old and 5-d-old chicks .
	manualset3
170863	7	413202	7	NULL	NULL	0	NULL	5-d-old chicks	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a positive effect of selenium supplementation of the maternal diet on glutathione concentration in the liver of 1-d-old and 5-d-old chicks .
	manualset3
170864	1	413203	7	NULL	NULL	0	NULL	positive relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a positive relationship between somatic cell count in milk and LAP expression .
	manualset3
170865	2	413203	7	NULL	NULL	0	NULL	somatic cell count	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a positive relationship between somatic cell count in milk and LAP expression .
	manualset3
170866	3	413203	7	NULL	NULL	0	NULL	milk	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a positive relationship between somatic cell count in milk and LAP expression .
	manualset3
170867	4	413203	7	NULL	NULL	0	NULL	LAP expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a positive relationship between somatic cell count in milk and LAP expression .
	manualset3
170868	1	413204	7	NULL	NULL	0	NULL	accumulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a preferential accumulation of the vitamin in the adrenals of the stress-imposed rats even though they were fed on a vitamin A-free diet .
	manualset3
170869	2	413204	7	NULL	NULL	0	NULL	 vitamin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a preferential accumulation of the vitamin in the adrenals of the stress-imposed rats even though they were fed on a vitamin A-free diet .
	manualset3
170870	3	413204	7	NULL	NULL	0	NULL	 adrenals	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a preferential accumulation of the vitamin in the adrenals of the stress-imposed rats even though they were fed on a vitamin A-free diet .
	manualset3
170871	4	413204	7	NULL	NULL	0	NULL	stress-imposed rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a preferential accumulation of the vitamin in the adrenals of the stress-imposed rats even though they were fed on a vitamin A-free diet .
	manualset3
170872	5	413204	7	NULL	NULL	0	NULL	vitamin A-free diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a preferential accumulation of the vitamin in the adrenals of the stress-imposed rats even though they were fed on a vitamin A-free diet .
	manualset3
170873	1	413205	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a relationship between smoking status and scores on the South Oaks Gambling Screen , and negative affect contributed to both gambling problems and tobacco dependence .
	manualset3
170874	2	413205	7	NULL	NULL	0	NULL	smoking status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a relationship between smoking status and scores on the South Oaks Gambling Screen , and negative affect contributed to both gambling problems and tobacco dependence .
	manualset3
170875	3	413205	7	NULL	NULL	0	NULL	scores	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a relationship between smoking status and scores on the South Oaks Gambling Screen , and negative affect contributed to both gambling problems and tobacco dependence .
	manualset3
170876	4	413205	7	NULL	NULL	0	NULL	South Oaks Gambling Screen	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a relationship between smoking status and scores on the South Oaks Gambling Screen , and negative affect contributed to both gambling problems and tobacco dependence .
	manualset3
170877	5	413205	7	NULL	NULL	NULL	NULL	negative affect	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There was a relationship between smoking status and scores on the South Oaks Gambling Screen , and negative affect contributed to both gambling problems and tobacco dependence .
	manualset3
170878	6	413205	7	NULL	NULL	NULL	NULL	gambling problems	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There was a relationship between smoking status and scores on the South Oaks Gambling Screen , and negative affect contributed to both gambling problems and tobacco dependence .
	manualset3
170879	7	413205	7	NULL	NULL	NULL	NULL	 tobacco dependence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There was a relationship between smoking status and scores on the South Oaks Gambling Screen , and negative affect contributed to both gambling problems and tobacco dependence .
	manualset3
170880	1	413206	7	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant correlation between both SBP and DBP to increasing height , weight and body mass index .
	manualset3
170882	2	413206	7	NULL	NULL	0	NULL	SBP	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant correlation between both SBP and DBP to increasing height , weight and body mass index .
	manualset3
170883	3	413206	7	NULL	NULL	0	NULL	DBP	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant correlation between both SBP and DBP to increasing height , weight and body mass index .
	manualset3
170884	4	413206	7	NULL	NULL	0	NULL	height	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant correlation between both SBP and DBP to increasing height , weight and body mass index .
	manualset3
170885	5	413206	7	NULL	NULL	0	NULL	 weight 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant correlation between both SBP and DBP to increasing height , weight and body mass index .
	manualset3
170886	6	413206	7	NULL	NULL	0	NULL	body mass index	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant correlation between both SBP and DBP to increasing height , weight and body mass index .
	manualset3
170887	1	413207	7	NULL	NULL	0	NULL	Active myocarditis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Active myocarditis was found in one case and postmyocarditic change in 9 cases .
	manualset3
170888	2	413207	7	NULL	NULL	0	NULL	one case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Active myocarditis was found in one case and postmyocarditic change in 9 cases .
	manualset3
170889	3	413207	7	NULL	NULL	0	NULL	postmyocarditic change 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Active myocarditis was found in one case and postmyocarditic change in 9 cases .
	manualset3
170890	4	413207	7	NULL	NULL	0	NULL	9 cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Active myocarditis was found in one case and postmyocarditic change in 9 cases .
	manualset3
170891	1	413208	7	NULL	NULL	0	NULL	 correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant correlation between log peak epinephrine and peak cortisol response ( r = 0.53 , p less than 0.0002 ) of the 46 subjects .
	manualset3
170892	2	413208	7	NULL	NULL	NULL	NULL	log peak epinephrine	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There was a significant correlation between log peak epinephrine and peak cortisol response ( r = 0.53 , p less than 0.0002 ) of the 46 subjects .
	manualset3
170893	3	413208	7	NULL	NULL	NULL	NULL	peak cortisol response	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There was a significant correlation between log peak epinephrine and peak cortisol response ( r = 0.53 , p less than 0.0002 ) of the 46 subjects .
	manualset3
170894	4	413208	7	NULL	NULL	0	NULL	 r = 0.53 , p less than 0.0002 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant correlation between log peak epinephrine and peak cortisol response ( r = 0.53 , p less than 0.0002 ) of the 46 subjects .
	manualset3
170895	5	413208	7	NULL	NULL	0	NULL	46 subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant correlation between log peak epinephrine and peak cortisol response ( r = 0.53 , p less than 0.0002 ) of the 46 subjects .
	manualset3
170896	1	413209	7	NULL	NULL	0	NULL	 correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant correlation between the angle of curvature and the difference in the cell wall extensibility between the convex and the concave sides .
	manualset3
170897	2	413209	7	NULL	NULL	0	NULL	angle of curvature	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant correlation between the angle of curvature and the difference in the cell wall extensibility between the convex and the concave sides .
	manualset3
170898	3	413209	7	NULL	NULL	0	NULL	 difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant correlation between the angle of curvature and the difference in the cell wall extensibility between the convex and the concave sides .
	manualset3
170899	4	413209	7	NULL	NULL	0	NULL	cell wall extensibility 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant correlation between the angle of curvature and the difference in the cell wall extensibility between the convex and the concave sides .
	manualset3
170900	5	413209	7	NULL	NULL	0	NULL	 convex side	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant correlation between the angle of curvature and the difference in the cell wall extensibility between the convex and the concave sides .
	manualset3
170901	6	413209	7	NULL	NULL	0	NULL	 concave sides	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant correlation between the angle of curvature and the difference in the cell wall extensibility between the convex and the concave sides .
	manualset3
170902	1	413210	7	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant difference between men and women in depth of the lumbar plexus ( median values , 85 vs 70 mm for men and women , respectively ) .
	manualset3
170903	2	413210	7	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant difference between men and women in depth of the lumbar plexus ( median values , 85 vs 70 mm for men and women , respectively ) .
	manualset3
170904	3	413210	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant difference between men and women in depth of the lumbar plexus ( median values , 85 vs 70 mm for men and women , respectively ) .
	manualset3
170905	4	413210	7	NULL	NULL	0	NULL	depth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant difference between men and women in depth of the lumbar plexus ( median values , 85 vs 70 mm for men and women , respectively ) .
	manualset3
170906	5	413210	7	NULL	NULL	0	NULL	lumbar plexus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant difference between men and women in depth of the lumbar plexus ( median values , 85 vs 70 mm for men and women , respectively ) .
	manualset3
170907	6	413210	7	NULL	NULL	0	NULL	median values , 85 vs 70 mm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant difference between men and women in depth of the lumbar plexus ( median values , 85 vs 70 mm for men and women , respectively ) .
	manualset3
170908	7	413210	7	NULL	NULL	0	NULL	 men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant difference between men and women in depth of the lumbar plexus ( median values , 85 vs 70 mm for men and women , respectively ) .
	manualset3
170909	8	413210	7	NULL	NULL	0	NULL	women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant difference between men and women in depth of the lumbar plexus ( median values , 85 vs 70 mm for men and women , respectively ) .
	manualset3
170910	1	413211	7	NULL	NULL	0	NULL	 increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant increase in HP values in samples from group 2c compared to 2a ( P = 0.018 ) .
	manualset3
170911	2	413211	7	NULL	NULL	0	NULL	HP values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant increase in HP values in samples from group 2c compared to 2a ( P = 0.018 ) .
	manualset3
170912	3	413211	7	NULL	NULL	0	NULL	samples	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant increase in HP values in samples from group 2c compared to 2a ( P = 0.018 ) .
	manualset3
170913	4	413211	7	NULL	NULL	0	NULL	group 2c	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant increase in HP values in samples from group 2c compared to 2a ( P = 0.018 ) .
	manualset3
170914	5	413211	7	NULL	NULL	0	NULL	2a	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant increase in HP values in samples from group 2c compared to 2a ( P = 0.018 ) .
	manualset3
170915	6	413211	7	NULL	NULL	0	NULL	P = 0.018	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant increase in HP values in samples from group 2c compared to 2a ( P = 0.018 ) .
	manualset3
171053	1	413212	7	NULL	NULL	0	NULL	inverse association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant inverse association between size of black area in AMs and lung function : each 1.0-microm2 increase in the area of the black material in AMs was associated with a 17.0 % ( 95 % confidence interval ( CI ) , 5.6 to 28.4 ) reduction in forced expiratory volume in one second ( FEV1 ) , a 12.9 % ( 95 % CI , 0.9 to 24.8 ) reduction in forced vital capacity ( FVC ) , and a 34.7 % ( 95 % CI , 11.3 to 58.1 ) reduction in forced expiratory flow between 25 % and 75 % of forced vital capacity ( FEF25 % -75 % ) .
	manualset3
171054	2	413212	7	NULL	NULL	0	NULL	size of black area	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant inverse association between size of black area in AMs and lung function : each 1.0-microm2 increase in the area of the black material in AMs was associated with a 17.0 % ( 95 % confidence interval ( CI ) , 5.6 to 28.4 ) reduction in forced expiratory volume in one second ( FEV1 ) , a 12.9 % ( 95 % CI , 0.9 to 24.8 ) reduction in forced vital capacity ( FVC ) , and a 34.7 % ( 95 % CI , 11.3 to 58.1 ) reduction in forced expiratory flow between 25 % and 75 % of forced vital capacity ( FEF25 % -75 % ) .
	manualset3
171055	3	413212	7	NULL	NULL	0	NULL	AMs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant inverse association between size of black area in AMs and lung function : each 1.0-microm2 increase in the area of the black material in AMs was associated with a 17.0 % ( 95 % confidence interval ( CI ) , 5.6 to 28.4 ) reduction in forced expiratory volume in one second ( FEV1 ) , a 12.9 % ( 95 % CI , 0.9 to 24.8 ) reduction in forced vital capacity ( FVC ) , and a 34.7 % ( 95 % CI , 11.3 to 58.1 ) reduction in forced expiratory flow between 25 % and 75 % of forced vital capacity ( FEF25 % -75 % ) .
	manualset3
171056	4	413212	7	NULL	NULL	0	NULL	lung function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant inverse association between size of black area in AMs and lung function : each 1.0-microm2 increase in the area of the black material in AMs was associated with a 17.0 % ( 95 % confidence interval ( CI ) , 5.6 to 28.4 ) reduction in forced expiratory volume in one second ( FEV1 ) , a 12.9 % ( 95 % CI , 0.9 to 24.8 ) reduction in forced vital capacity ( FVC ) , and a 34.7 % ( 95 % CI , 11.3 to 58.1 ) reduction in forced expiratory flow between 25 % and 75 % of forced vital capacity ( FEF25 % -75 % ) .
	manualset3
171057	5	413212	7	NULL	NULL	0	NULL	1.0-microm2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant inverse association between size of black area in AMs and lung function : each 1.0-microm2 increase in the area of the black material in AMs was associated with a 17.0 % ( 95 % confidence interval ( CI ) , 5.6 to 28.4 ) reduction in forced expiratory volume in one second ( FEV1 ) , a 12.9 % ( 95 % CI , 0.9 to 24.8 ) reduction in forced vital capacity ( FVC ) , and a 34.7 % ( 95 % CI , 11.3 to 58.1 ) reduction in forced expiratory flow between 25 % and 75 % of forced vital capacity ( FEF25 % -75 % ) .
	manualset3
171058	6	413212	7	NULL	NULL	0	NULL	increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant inverse association between size of black area in AMs and lung function : each 1.0-microm2 increase in the area of the black material in AMs was associated with a 17.0 % ( 95 % confidence interval ( CI ) , 5.6 to 28.4 ) reduction in forced expiratory volume in one second ( FEV1 ) , a 12.9 % ( 95 % CI , 0.9 to 24.8 ) reduction in forced vital capacity ( FVC ) , and a 34.7 % ( 95 % CI , 11.3 to 58.1 ) reduction in forced expiratory flow between 25 % and 75 % of forced vital capacity ( FEF25 % -75 % ) .
	manualset3
171059	7	413212	7	NULL	NULL	0	NULL	area	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant inverse association between size of black area in AMs and lung function : each 1.0-microm2 increase in the area of the black material in AMs was associated with a 17.0 % ( 95 % confidence interval ( CI ) , 5.6 to 28.4 ) reduction in forced expiratory volume in one second ( FEV1 ) , a 12.9 % ( 95 % CI , 0.9 to 24.8 ) reduction in forced vital capacity ( FVC ) , and a 34.7 % ( 95 % CI , 11.3 to 58.1 ) reduction in forced expiratory flow between 25 % and 75 % of forced vital capacity ( FEF25 % -75 % ) .
	manualset3
171060	8	413212	7	NULL	NULL	0	NULL	black material	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant inverse association between size of black area in AMs and lung function : each 1.0-microm2 increase in the area of the black material in AMs was associated with a 17.0 % ( 95 % confidence interval ( CI ) , 5.6 to 28.4 ) reduction in forced expiratory volume in one second ( FEV1 ) , a 12.9 % ( 95 % CI , 0.9 to 24.8 ) reduction in forced vital capacity ( FVC ) , and a 34.7 % ( 95 % CI , 11.3 to 58.1 ) reduction in forced expiratory flow between 25 % and 75 % of forced vital capacity ( FEF25 % -75 % ) .
	manualset3
171061	9	413212	7	NULL	NULL	0	NULL	AMs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant inverse association between size of black area in AMs and lung function : each 1.0-microm2 increase in the area of the black material in AMs was associated with a 17.0 % ( 95 % confidence interval ( CI ) , 5.6 to 28.4 ) reduction in forced expiratory volume in one second ( FEV1 ) , a 12.9 % ( 95 % CI , 0.9 to 24.8 ) reduction in forced vital capacity ( FVC ) , and a 34.7 % ( 95 % CI , 11.3 to 58.1 ) reduction in forced expiratory flow between 25 % and 75 % of forced vital capacity ( FEF25 % -75 % ) .
	manualset3
171062	10	413212	7	NULL	NULL	NULL	NULL	17.0 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There was a significant inverse association between size of black area in AMs and lung function : each 1.0-microm2 increase in the area of the black material in AMs was associated with a 17.0 % ( 95 % confidence interval ( CI ) , 5.6 to 28.4 ) reduction in forced expiratory volume in one second ( FEV1 ) , a 12.9 % ( 95 % CI , 0.9 to 24.8 ) reduction in forced vital capacity ( FVC ) , and a 34.7 % ( 95 % CI , 11.3 to 58.1 ) reduction in forced expiratory flow between 25 % and 75 % of forced vital capacity ( FEF25 % -75 % ) .
	manualset3
171063	11	413212	7	NULL	NULL	NULL	NULL	 95 % confidence interval ( CI ) , 5.6 to 28.4	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There was a significant inverse association between size of black area in AMs and lung function : each 1.0-microm2 increase in the area of the black material in AMs was associated with a 17.0 % ( 95 % confidence interval ( CI ) , 5.6 to 28.4 ) reduction in forced expiratory volume in one second ( FEV1 ) , a 12.9 % ( 95 % CI , 0.9 to 24.8 ) reduction in forced vital capacity ( FVC ) , and a 34.7 % ( 95 % CI , 11.3 to 58.1 ) reduction in forced expiratory flow between 25 % and 75 % of forced vital capacity ( FEF25 % -75 % ) .
	manualset3
171065	13	413212	7	NULL	NULL	0	NULL	 reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant inverse association between size of black area in AMs and lung function : each 1.0-microm2 increase in the area of the black material in AMs was associated with a 17.0 % ( 95 % confidence interval ( CI ) , 5.6 to 28.4 ) reduction in forced expiratory volume in one second ( FEV1 ) , a 12.9 % ( 95 % CI , 0.9 to 24.8 ) reduction in forced vital capacity ( FVC ) , and a 34.7 % ( 95 % CI , 11.3 to 58.1 ) reduction in forced expiratory flow between 25 % and 75 % of forced vital capacity ( FEF25 % -75 % ) .
	manualset3
171066	14	413212	7	NULL	NULL	NULL	NULL	forced expiratory volume in one second ( FEV1 )	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There was a significant inverse association between size of black area in AMs and lung function : each 1.0-microm2 increase in the area of the black material in AMs was associated with a 17.0 % ( 95 % confidence interval ( CI ) , 5.6 to 28.4 ) reduction in forced expiratory volume in one second ( FEV1 ) , a 12.9 % ( 95 % CI , 0.9 to 24.8 ) reduction in forced vital capacity ( FVC ) , and a 34.7 % ( 95 % CI , 11.3 to 58.1 ) reduction in forced expiratory flow between 25 % and 75 % of forced vital capacity ( FEF25 % -75 % ) .
	manualset3
171067	15	413212	7	NULL	NULL	0	NULL	12.9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant inverse association between size of black area in AMs and lung function : each 1.0-microm2 increase in the area of the black material in AMs was associated with a 17.0 % ( 95 % confidence interval ( CI ) , 5.6 to 28.4 ) reduction in forced expiratory volume in one second ( FEV1 ) , a 12.9 % ( 95 % CI , 0.9 to 24.8 ) reduction in forced vital capacity ( FVC ) , and a 34.7 % ( 95 % CI , 11.3 to 58.1 ) reduction in forced expiratory flow between 25 % and 75 % of forced vital capacity ( FEF25 % -75 % ) .
	manualset3
171068	16	413212	7	NULL	NULL	NULL	NULL	95 % CI , 0.9 to 24.8	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There was a significant inverse association between size of black area in AMs and lung function : each 1.0-microm2 increase in the area of the black material in AMs was associated with a 17.0 % ( 95 % confidence interval ( CI ) , 5.6 to 28.4 ) reduction in forced expiratory volume in one second ( FEV1 ) , a 12.9 % ( 95 % CI , 0.9 to 24.8 ) reduction in forced vital capacity ( FVC ) , and a 34.7 % ( 95 % CI , 11.3 to 58.1 ) reduction in forced expiratory flow between 25 % and 75 % of forced vital capacity ( FEF25 % -75 % ) .
	manualset3
171069	17	413212	7	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant inverse association between size of black area in AMs and lung function : each 1.0-microm2 increase in the area of the black material in AMs was associated with a 17.0 % ( 95 % confidence interval ( CI ) , 5.6 to 28.4 ) reduction in forced expiratory volume in one second ( FEV1 ) , a 12.9 % ( 95 % CI , 0.9 to 24.8 ) reduction in forced vital capacity ( FVC ) , and a 34.7 % ( 95 % CI , 11.3 to 58.1 ) reduction in forced expiratory flow between 25 % and 75 % of forced vital capacity ( FEF25 % -75 % ) .
	manualset3
171070	18	413212	7	NULL	NULL	0	NULL	forced vital capacity ( FVC )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant inverse association between size of black area in AMs and lung function : each 1.0-microm2 increase in the area of the black material in AMs was associated with a 17.0 % ( 95 % confidence interval ( CI ) , 5.6 to 28.4 ) reduction in forced expiratory volume in one second ( FEV1 ) , a 12.9 % ( 95 % CI , 0.9 to 24.8 ) reduction in forced vital capacity ( FVC ) , and a 34.7 % ( 95 % CI , 11.3 to 58.1 ) reduction in forced expiratory flow between 25 % and 75 % of forced vital capacity ( FEF25 % -75 % ) .
	manualset3
171071	19	413212	7	NULL	NULL	0	NULL	34.7 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant inverse association between size of black area in AMs and lung function : each 1.0-microm2 increase in the area of the black material in AMs was associated with a 17.0 % ( 95 % confidence interval ( CI ) , 5.6 to 28.4 ) reduction in forced expiratory volume in one second ( FEV1 ) , a 12.9 % ( 95 % CI , 0.9 to 24.8 ) reduction in forced vital capacity ( FVC ) , and a 34.7 % ( 95 % CI , 11.3 to 58.1 ) reduction in forced expiratory flow between 25 % and 75 % of forced vital capacity ( FEF25 % -75 % ) .
	manualset3
171072	20	413212	7	NULL	NULL	NULL	NULL	95 % CI , 11.3 to 58.1	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There was a significant inverse association between size of black area in AMs and lung function : each 1.0-microm2 increase in the area of the black material in AMs was associated with a 17.0 % ( 95 % confidence interval ( CI ) , 5.6 to 28.4 ) reduction in forced expiratory volume in one second ( FEV1 ) , a 12.9 % ( 95 % CI , 0.9 to 24.8 ) reduction in forced vital capacity ( FVC ) , and a 34.7 % ( 95 % CI , 11.3 to 58.1 ) reduction in forced expiratory flow between 25 % and 75 % of forced vital capacity ( FEF25 % -75 % ) .
	manualset3
171074	22	413212	7	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant inverse association between size of black area in AMs and lung function : each 1.0-microm2 increase in the area of the black material in AMs was associated with a 17.0 % ( 95 % confidence interval ( CI ) , 5.6 to 28.4 ) reduction in forced expiratory volume in one second ( FEV1 ) , a 12.9 % ( 95 % CI , 0.9 to 24.8 ) reduction in forced vital capacity ( FVC ) , and a 34.7 % ( 95 % CI , 11.3 to 58.1 ) reduction in forced expiratory flow between 25 % and 75 % of forced vital capacity ( FEF25 % -75 % ) .
	manualset3
171075	23	413212	7	NULL	NULL	0	NULL	forced expiratory flow	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant inverse association between size of black area in AMs and lung function : each 1.0-microm2 increase in the area of the black material in AMs was associated with a 17.0 % ( 95 % confidence interval ( CI ) , 5.6 to 28.4 ) reduction in forced expiratory volume in one second ( FEV1 ) , a 12.9 % ( 95 % CI , 0.9 to 24.8 ) reduction in forced vital capacity ( FVC ) , and a 34.7 % ( 95 % CI , 11.3 to 58.1 ) reduction in forced expiratory flow between 25 % and 75 % of forced vital capacity ( FEF25 % -75 % ) .
	manualset3
171076	24	413212	7	NULL	NULL	0	NULL	 25 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant inverse association between size of black area in AMs and lung function : each 1.0-microm2 increase in the area of the black material in AMs was associated with a 17.0 % ( 95 % confidence interval ( CI ) , 5.6 to 28.4 ) reduction in forced expiratory volume in one second ( FEV1 ) , a 12.9 % ( 95 % CI , 0.9 to 24.8 ) reduction in forced vital capacity ( FVC ) , and a 34.7 % ( 95 % CI , 11.3 to 58.1 ) reduction in forced expiratory flow between 25 % and 75 % of forced vital capacity ( FEF25 % -75 % ) .
	manualset3
171077	25	413212	7	NULL	NULL	0	NULL	75 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant inverse association between size of black area in AMs and lung function : each 1.0-microm2 increase in the area of the black material in AMs was associated with a 17.0 % ( 95 % confidence interval ( CI ) , 5.6 to 28.4 ) reduction in forced expiratory volume in one second ( FEV1 ) , a 12.9 % ( 95 % CI , 0.9 to 24.8 ) reduction in forced vital capacity ( FVC ) , and a 34.7 % ( 95 % CI , 11.3 to 58.1 ) reduction in forced expiratory flow between 25 % and 75 % of forced vital capacity ( FEF25 % -75 % ) .
	manualset3
171078	26	413212	7	NULL	NULL	0	NULL	forced vital capacity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant inverse association between size of black area in AMs and lung function : each 1.0-microm2 increase in the area of the black material in AMs was associated with a 17.0 % ( 95 % confidence interval ( CI ) , 5.6 to 28.4 ) reduction in forced expiratory volume in one second ( FEV1 ) , a 12.9 % ( 95 % CI , 0.9 to 24.8 ) reduction in forced vital capacity ( FVC ) , and a 34.7 % ( 95 % CI , 11.3 to 58.1 ) reduction in forced expiratory flow between 25 % and 75 % of forced vital capacity ( FEF25 % -75 % ) .
	manualset3
171079	27	413212	7	NULL	NULL	0	NULL	FEF25 % -75 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant inverse association between size of black area in AMs and lung function : each 1.0-microm2 increase in the area of the black material in AMs was associated with a 17.0 % ( 95 % confidence interval ( CI ) , 5.6 to 28.4 ) reduction in forced expiratory volume in one second ( FEV1 ) , a 12.9 % ( 95 % CI , 0.9 to 24.8 ) reduction in forced vital capacity ( FVC ) , and a 34.7 % ( 95 % CI , 11.3 to 58.1 ) reduction in forced expiratory flow between 25 % and 75 % of forced vital capacity ( FEF25 % -75 % ) .
	manualset3
171080	1	413213	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant relationship between food refusal and hypersensitivity ( p = 0.021 ) .
	manualset3
171081	2	413213	7	NULL	NULL	0	NULL	food refusal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant relationship between food refusal and hypersensitivity ( p = 0.021 ) .
	manualset3
171082	3	413213	7	NULL	NULL	0	NULL	 hypersensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant relationship between food refusal and hypersensitivity ( p = 0.021 ) .
	manualset3
171083	4	413213	7	NULL	NULL	0	NULL	p = 0.021	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significant relationship between food refusal and hypersensitivity ( p = 0.021 ) .
	manualset3
171084	1	413214	7	NULL	NULL	0	NULL	P & lt ; 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significantly higher ( P & lt ; 0.01 ) incidence of associated upper extremity injury in the group with RSD ( 75 % ) .
	manualset3
171085	2	413214	7	NULL	NULL	0	NULL	 incidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significantly higher ( P & lt ; 0.01 ) incidence of associated upper extremity injury in the group with RSD ( 75 % ) .
	manualset3
171086	3	413214	7	NULL	NULL	0	NULL	upper extremity injury 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significantly higher ( P & lt ; 0.01 ) incidence of associated upper extremity injury in the group with RSD ( 75 % ) .
	manualset3
171087	4	413214	7	NULL	NULL	0	NULL	group	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significantly higher ( P & lt ; 0.01 ) incidence of associated upper extremity injury in the group with RSD ( 75 % ) .
	manualset3
171088	5	413214	7	NULL	NULL	0	NULL	RSD ( 75 % )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a significantly higher ( P & lt ; 0.01 ) incidence of associated upper extremity injury in the group with RSD ( 75 % ) .
	manualset3
171089	1	413215	7	NULL	NULL	0	NULL	Active oxygen generation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Active oxygen generation in gamma-irradiated whole seedlings of Cicer arietinum L .
	manualset3
171090	2	413215	7	NULL	NULL	0	NULL	 gamma-irradiated whole seedlings	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Active oxygen generation in gamma-irradiated whole seedlings of Cicer arietinum L .
	manualset3
171091	3	413215	7	NULL	NULL	0	NULL	Cicer arietinum L	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Active oxygen generation in gamma-irradiated whole seedlings of Cicer arietinum L .
	manualset3
171092	1	413216	7	NULL	NULL	0	NULL	 similar contrast	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a similar contrast between women from Haiti and those from the French Antilles ; ( b ) drug abuse plays a major role in the other seropositive women : 70 p. 100 were drug addict and 15 p. 100 had been contaminated by male drug addicts .
	manualset3
171093	2	413216	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a similar contrast between women from Haiti and those from the French Antilles ; ( b ) drug abuse plays a major role in the other seropositive women : 70 p. 100 were drug addict and 15 p. 100 had been contaminated by male drug addicts .
	manualset3
171094	3	413216	7	NULL	NULL	0	NULL	Haiti	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a similar contrast between women from Haiti and those from the French Antilles ; ( b ) drug abuse plays a major role in the other seropositive women : 70 p. 100 were drug addict and 15 p. 100 had been contaminated by male drug addicts .
	manualset3
171095	4	413216	7	NULL	NULL	0	NULL	French Antilles	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a similar contrast between women from Haiti and those from the French Antilles ; ( b ) drug abuse plays a major role in the other seropositive women : 70 p. 100 were drug addict and 15 p. 100 had been contaminated by male drug addicts .
	manualset3
171096	5	413216	7	NULL	NULL	0	NULL	 drug abuse	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a similar contrast between women from Haiti and those from the French Antilles ; ( b ) drug abuse plays a major role in the other seropositive women : 70 p. 100 were drug addict and 15 p. 100 had been contaminated by male drug addicts .
	manualset3
171097	6	413216	7	NULL	NULL	0	NULL	major role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a similar contrast between women from Haiti and those from the French Antilles ; ( b ) drug abuse plays a major role in the other seropositive women : 70 p. 100 were drug addict and 15 p. 100 had been contaminated by male drug addicts .
	manualset3
171098	7	413216	7	NULL	NULL	0	NULL	seropositive women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a similar contrast between women from Haiti and those from the French Antilles ; ( b ) drug abuse plays a major role in the other seropositive women : 70 p. 100 were drug addict and 15 p. 100 had been contaminated by male drug addicts .
	manualset3
171099	8	413216	7	NULL	NULL	0	NULL	70 p. 100	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a similar contrast between women from Haiti and those from the French Antilles ; ( b ) drug abuse plays a major role in the other seropositive women : 70 p. 100 were drug addict and 15 p. 100 had been contaminated by male drug addicts .
	manualset3
171100	9	413216	7	NULL	NULL	0	NULL	drug addict 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a similar contrast between women from Haiti and those from the French Antilles ; ( b ) drug abuse plays a major role in the other seropositive women : 70 p. 100 were drug addict and 15 p. 100 had been contaminated by male drug addicts .
	manualset3
171101	10	413216	7	NULL	NULL	0	NULL	15 p. 100	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a similar contrast between women from Haiti and those from the French Antilles ; ( b ) drug abuse plays a major role in the other seropositive women : 70 p. 100 were drug addict and 15 p. 100 had been contaminated by male drug addicts .
	manualset3
171102	11	413216	7	NULL	NULL	0	NULL	male drug addicts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a similar contrast between women from Haiti and those from the French Antilles ; ( b ) drug abuse plays a major role in the other seropositive women : 70 p. 100 were drug addict and 15 p. 100 had been contaminated by male drug addicts .
	manualset3
171153	1	413217	7	NULL	NULL	0	NULL	correlation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a statistically significant correlation between maternal urinary and umbilical cord serum level of cotinine ( P & lt ; 0.001 , r = 0.58 ) .
	manualset3
171154	2	413217	7	NULL	NULL	0	NULL	maternal urinary level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a statistically significant correlation between maternal urinary and umbilical cord serum level of cotinine ( P & lt ; 0.001 , r = 0.58 ) .
	manualset3
171155	3	413217	7	NULL	NULL	0	NULL	 umbilical cord serum level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a statistically significant correlation between maternal urinary and umbilical cord serum level of cotinine ( P & lt ; 0.001 , r = 0.58 ) .
	manualset3
171156	4	413217	7	NULL	NULL	0	NULL	cotinine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a statistically significant correlation between maternal urinary and umbilical cord serum level of cotinine ( P & lt ; 0.001 , r = 0.58 ) .
	manualset3
171157	5	413217	7	NULL	NULL	0	NULL	P & lt ; 0.001 , r = 0.58	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a statistically significant correlation between maternal urinary and umbilical cord serum level of cotinine ( P & lt ; 0.001 , r = 0.58 ) .
	manualset3
171158	1	413218	7	NULL	NULL	0	NULL	fall	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a statistically significant fall of serum TC ( P = 0.002 ) , LDL-C ( P = 0.016 ) , and triglyceride ( P = 0.029 ) levels at the end of periods A and B. Kidney and liver function did not change .
	manualset3
171159	2	413218	7	NULL	NULL	0	NULL	serum TC	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a statistically significant fall of serum TC ( P = 0.002 ) , LDL-C ( P = 0.016 ) , and triglyceride ( P = 0.029 ) levels at the end of periods A and B. Kidney and liver function did not change .
	manualset3
171160	3	413218	7	NULL	NULL	0	NULL	 P = 0.002	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a statistically significant fall of serum TC ( P = 0.002 ) , LDL-C ( P = 0.016 ) , and triglyceride ( P = 0.029 ) levels at the end of periods A and B. Kidney and liver function did not change .
	manualset3
171161	4	413218	7	NULL	NULL	0	NULL	LDL-C	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a statistically significant fall of serum TC ( P = 0.002 ) , LDL-C ( P = 0.016 ) , and triglyceride ( P = 0.029 ) levels at the end of periods A and B. Kidney and liver function did not change .
	manualset3
171162	5	413218	7	NULL	NULL	0	NULL	 P = 0.016	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a statistically significant fall of serum TC ( P = 0.002 ) , LDL-C ( P = 0.016 ) , and triglyceride ( P = 0.029 ) levels at the end of periods A and B. Kidney and liver function did not change .
	manualset3
171163	6	413218	7	NULL	NULL	NULL	NULL	 triglyceride levels	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There was a statistically significant fall of serum TC ( P = 0.002 ) , LDL-C ( P = 0.016 ) , and triglyceride ( P = 0.029 ) levels at the end of periods A and B. Kidney and liver function did not change .
	manualset3
171164	7	413218	7	NULL	NULL	0	NULL	 P = 0.029	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a statistically significant fall of serum TC ( P = 0.002 ) , LDL-C ( P = 0.016 ) , and triglyceride ( P = 0.029 ) levels at the end of periods A and B. Kidney and liver function did not change .
	manualset3
171165	8	413218	7	NULL	NULL	0	NULL	end of periods A	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a statistically significant fall of serum TC ( P = 0.002 ) , LDL-C ( P = 0.016 ) , and triglyceride ( P = 0.029 ) levels at the end of periods A and B. Kidney and liver function did not change .
	manualset3
171166	9	413218	7	NULL	NULL	0	NULL	end of periods B	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a statistically significant fall of serum TC ( P = 0.002 ) , LDL-C ( P = 0.016 ) , and triglyceride ( P = 0.029 ) levels at the end of periods A and B. Kidney and liver function did not change .
	manualset3
171167	10	413218	7	NULL	NULL	0	NULL	 Kidney function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a statistically significant fall of serum TC ( P = 0.002 ) , LDL-C ( P = 0.016 ) , and triglyceride ( P = 0.029 ) levels at the end of periods A and B. Kidney and liver function did not change .
	manualset3
171168	11	413218	7	NULL	NULL	0	NULL	liver function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a statistically significant fall of serum TC ( P = 0.002 ) , LDL-C ( P = 0.016 ) , and triglyceride ( P = 0.029 ) levels at the end of periods A and B. Kidney and liver function did not change .
	manualset3
171215	1	413219	7	NULL	NULL	0	NULL	 improvement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a statistically significant improvement in the proportion of biopsies positive for cancer , reflecting reduction in unnecessary biopsies , but the pre-existing annual improvement in reducing postoperative stays was not accelerated .
	manualset3
171216	2	413219	7	NULL	NULL	0	NULL	proportion	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a statistically significant improvement in the proportion of biopsies positive for cancer , reflecting reduction in unnecessary biopsies , but the pre-existing annual improvement in reducing postoperative stays was not accelerated .
	manualset3
171217	3	413219	7	NULL	NULL	0	NULL	biopsies 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a statistically significant improvement in the proportion of biopsies positive for cancer , reflecting reduction in unnecessary biopsies , but the pre-existing annual improvement in reducing postoperative stays was not accelerated .
	manualset3
171218	4	413219	7	NULL	NULL	0	NULL	cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a statistically significant improvement in the proportion of biopsies positive for cancer , reflecting reduction in unnecessary biopsies , but the pre-existing annual improvement in reducing postoperative stays was not accelerated .
	manualset3
171219	5	413219	7	NULL	NULL	0	NULL	reduction	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a statistically significant improvement in the proportion of biopsies positive for cancer , reflecting reduction in unnecessary biopsies , but the pre-existing annual improvement in reducing postoperative stays was not accelerated .
	manualset3
171220	6	413219	7	NULL	NULL	0	NULL	 biopsies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a statistically significant improvement in the proportion of biopsies positive for cancer , reflecting reduction in unnecessary biopsies , but the pre-existing annual improvement in reducing postoperative stays was not accelerated .
	manualset3
171221	7	413219	7	NULL	NULL	0	NULL	pre-existing annual improvement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a statistically significant improvement in the proportion of biopsies positive for cancer , reflecting reduction in unnecessary biopsies , but the pre-existing annual improvement in reducing postoperative stays was not accelerated .
	manualset3
171222	8	413219	7	NULL	NULL	0	NULL	postoperative stays 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a statistically significant improvement in the proportion of biopsies positive for cancer , reflecting reduction in unnecessary biopsies , but the pre-existing annual improvement in reducing postoperative stays was not accelerated .
	manualset3
171223	1	413220	7	NULL	NULL	0	NULL	trend 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a trend in favor of halobetasol propionate in the cutaneous vasoconstriction assay performed in volunteers with ethanol solutions of halobetasol propionate and clobetasol 17-propionate .
	manualset3
171224	2	413220	7	NULL	NULL	0	NULL	halobetasol propionate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a trend in favor of halobetasol propionate in the cutaneous vasoconstriction assay performed in volunteers with ethanol solutions of halobetasol propionate and clobetasol 17-propionate .
	manualset3
171225	3	413220	7	NULL	NULL	0	NULL	cutaneous vasoconstriction assay	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a trend in favor of halobetasol propionate in the cutaneous vasoconstriction assay performed in volunteers with ethanol solutions of halobetasol propionate and clobetasol 17-propionate .
	manualset3
171226	4	413220	7	NULL	NULL	0	NULL	volunteers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a trend in favor of halobetasol propionate in the cutaneous vasoconstriction assay performed in volunteers with ethanol solutions of halobetasol propionate and clobetasol 17-propionate .
	manualset3
171227	5	413220	7	NULL	NULL	0	NULL	ethanol solutions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a trend in favor of halobetasol propionate in the cutaneous vasoconstriction assay performed in volunteers with ethanol solutions of halobetasol propionate and clobetasol 17-propionate .
	manualset3
171228	6	413220	7	NULL	NULL	0	NULL	halobetasol propionate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a trend in favor of halobetasol propionate in the cutaneous vasoconstriction assay performed in volunteers with ethanol solutions of halobetasol propionate and clobetasol 17-propionate .
	manualset3
171229	7	413220	7	NULL	NULL	0	NULL	clobetasol 17-propionate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a trend in favor of halobetasol propionate in the cutaneous vasoconstriction assay performed in volunteers with ethanol solutions of halobetasol propionate and clobetasol 17-propionate .
	manualset3
171230	1	413221	7	NULL	NULL	0	NULL	good positive correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a very good positive correlation between the agglutinating activity of abrin-a and development of apoptosis to DNA fragmentation .
	manualset3
171231	2	413221	7	NULL	NULL	0	NULL	agglutinating activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a very good positive correlation between the agglutinating activity of abrin-a and development of apoptosis to DNA fragmentation .
	manualset3
171232	3	413221	7	NULL	NULL	0	NULL	abrin-a	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a very good positive correlation between the agglutinating activity of abrin-a and development of apoptosis to DNA fragmentation .
	manualset3
171233	4	413221	7	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a very good positive correlation between the agglutinating activity of abrin-a and development of apoptosis to DNA fragmentation .
	manualset3
171234	5	413221	7	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a very good positive correlation between the agglutinating activity of abrin-a and development of apoptosis to DNA fragmentation .
	manualset3
171235	6	413221	7	NULL	NULL	0	NULL	 DNA fragmentation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was a very good positive correlation between the agglutinating activity of abrin-a and development of apoptosis to DNA fragmentation .
	manualset3
171236	1	413222	7	NULL	NULL	0	NULL	 change 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was also a change in the distribution of albumin from the extravascular to the intravascular pool and a significant increase in the plasma and blood volumes of infected calves although the blood and albumin loss via the gastrointestinal tract recorded in this study was similar in both groups .
	manualset3
171237	2	413222	7	NULL	NULL	0	NULL	 distribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was also a change in the distribution of albumin from the extravascular to the intravascular pool and a significant increase in the plasma and blood volumes of infected calves although the blood and albumin loss via the gastrointestinal tract recorded in this study was similar in both groups .
	manualset3
171238	3	413222	7	NULL	NULL	0	NULL	 albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	There was also a change in the distribution of albumin from the extravascular to the intravascular pool and a significant increase in the plasma and blood volumes of infected calves although the blood and albumin loss via the gastrointestinal tract recorded in this study was similar in both groups .
	manualset3
171239	4	413222	7	NULL	NULL	0	NULL	extravascular pool	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There was also a change in the distribution of albumin from the extravascular to the intravascular pool and a significant increase in the plasma and blood volumes of infected calves although the blood and albumin loss via the gastrointestinal tract recorded in this study was similar in both groups .
	manualset3
171240	5	413222	7	NULL	NULL	0	NULL	intravascular pool 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There was also a change in the distribution of albumin from the extravascular to the intravascular pool and a significant increase in the plasma and blood volumes of infected calves although the blood and albumin loss via the gastrointestinal tract recorded in this study was similar in both groups .
	manualset3
171241	6	413222	7	NULL	NULL	0	NULL	 increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was also a change in the distribution of albumin from the extravascular to the intravascular pool and a significant increase in the plasma and blood volumes of infected calves although the blood and albumin loss via the gastrointestinal tract recorded in this study was similar in both groups .
	manualset3
171242	7	413222	7	NULL	NULL	0	NULL	plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There was also a change in the distribution of albumin from the extravascular to the intravascular pool and a significant increase in the plasma and blood volumes of infected calves although the blood and albumin loss via the gastrointestinal tract recorded in this study was similar in both groups .
	manualset3
171243	8	413222	7	NULL	NULL	0	NULL	 blood volumes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was also a change in the distribution of albumin from the extravascular to the intravascular pool and a significant increase in the plasma and blood volumes of infected calves although the blood and albumin loss via the gastrointestinal tract recorded in this study was similar in both groups .
	manualset3
171244	9	413222	7	NULL	NULL	0	NULL	infected calves	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	There was also a change in the distribution of albumin from the extravascular to the intravascular pool and a significant increase in the plasma and blood volumes of infected calves although the blood and albumin loss via the gastrointestinal tract recorded in this study was similar in both groups .
	manualset3
171245	10	413222	7	NULL	NULL	0	NULL	blood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There was also a change in the distribution of albumin from the extravascular to the intravascular pool and a significant increase in the plasma and blood volumes of infected calves although the blood and albumin loss via the gastrointestinal tract recorded in this study was similar in both groups .
	manualset3
171246	11	413222	7	NULL	NULL	0	NULL	albumin loss 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was also a change in the distribution of albumin from the extravascular to the intravascular pool and a significant increase in the plasma and blood volumes of infected calves although the blood and albumin loss via the gastrointestinal tract recorded in this study was similar in both groups .
	manualset3
171247	12	413222	7	NULL	NULL	0	NULL	 gastrointestinal tract 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There was also a change in the distribution of albumin from the extravascular to the intravascular pool and a significant increase in the plasma and blood volumes of infected calves although the blood and albumin loss via the gastrointestinal tract recorded in this study was similar in both groups .
	manualset3
171248	13	413222	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was also a change in the distribution of albumin from the extravascular to the intravascular pool and a significant increase in the plasma and blood volumes of infected calves although the blood and albumin loss via the gastrointestinal tract recorded in this study was similar in both groups .
	manualset3
171249	14	413222	7	NULL	NULL	0	NULL	similar	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was also a change in the distribution of albumin from the extravascular to the intravascular pool and a significant increase in the plasma and blood volumes of infected calves although the blood and albumin loss via the gastrointestinal tract recorded in this study was similar in both groups .
	manualset3
171250	15	413222	7	NULL	NULL	NULL	NULL	groups	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There was also a change in the distribution of albumin from the extravascular to the intravascular pool and a significant increase in the plasma and blood volumes of infected calves although the blood and albumin loss via the gastrointestinal tract recorded in this study was similar in both groups .
	manualset3
171251	1	413223	7	NULL	NULL	0	NULL	 decrease	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was also a decrease in blood pressure readings in our study subjects .
	manualset3
171252	2	413223	7	NULL	NULL	0	NULL	 blood pressure readings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was also a decrease in blood pressure readings in our study subjects .
	manualset3
171253	3	413223	7	NULL	NULL	0	NULL	study subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There was also a decrease in blood pressure readings in our study subjects .
	manualset3
171254	1	413224	7	NULL	NULL	0	NULL	 strong relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was also a strong relationship between increased infarct size and decreased perfusion .
	manualset3
171255	2	413224	7	NULL	NULL	0	NULL	 increased infarct size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was also a strong relationship between increased infarct size and decreased perfusion .
	manualset3
171256	3	413224	7	NULL	NULL	0	NULL	 decreased perfusion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was also a strong relationship between increased infarct size and decreased perfusion .
	manualset3
171257	1	413225	7	NULL	NULL	0	NULL	 no correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was also no correlation between the expression of Oct-2 and levels of immunoglobulin-specific messenger RNAs .
	manualset3
171258	2	413225	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was also no correlation between the expression of Oct-2 and levels of immunoglobulin-specific messenger RNAs .
	manualset3
171259	3	413225	7	NULL	NULL	0	NULL	Oct-2	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	There was also no correlation between the expression of Oct-2 and levels of immunoglobulin-specific messenger RNAs .
	manualset3
171260	4	413225	7	NULL	NULL	0	NULL	 levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was also no correlation between the expression of Oct-2 and levels of immunoglobulin-specific messenger RNAs .
	manualset3
171261	5	413225	7	NULL	NULL	0	NULL	 immunoglobulin-specific messenger RNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	There was also no correlation between the expression of Oct-2 and levels of immunoglobulin-specific messenger RNAs .
	manualset3
171262	1	413226	7	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was an association between histologic type of carcinoma in LN metastasis and the predominant histologic type of the primary tumor .
	manualset3
171263	2	413226	7	NULL	NULL	0	NULL	 histologic type	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was an association between histologic type of carcinoma in LN metastasis and the predominant histologic type of the primary tumor .
	manualset3
171264	3	413226	7	NULL	NULL	0	NULL	carcinoma in LN metastasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was an association between histologic type of carcinoma in LN metastasis and the predominant histologic type of the primary tumor .
	manualset3
171265	4	413226	7	NULL	NULL	0	NULL	histologic type	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was an association between histologic type of carcinoma in LN metastasis and the predominant histologic type of the primary tumor .
	manualset3
171266	5	413226	7	NULL	NULL	0	NULL	primary tumor	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There was an association between histologic type of carcinoma in LN metastasis and the predominant histologic type of the primary tumor .
	manualset3
171267	1	413227	7	NULL	NULL	0	NULL	overall increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was an overall increase in disability ( Steinbrocker ) and the use of walking aids in the group but 57 patients ( 13.7 % ) improved , 38 of whom had undergone joint surgery .
	manualset3
171268	2	413227	7	NULL	NULL	NULL	NULL	 disability ( Steinbrocker ) 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There was an overall increase in disability ( Steinbrocker ) and the use of walking aids in the group but 57 patients ( 13.7 % ) improved , 38 of whom had undergone joint surgery .
	manualset3
171269	3	413227	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There was an overall increase in disability ( Steinbrocker ) and the use of walking aids in the group but 57 patients ( 13.7 % ) improved , 38 of whom had undergone joint surgery .
	manualset3
171270	4	413227	7	NULL	NULL	0	NULL	 walking aids	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	There was an overall increase in disability ( Steinbrocker ) and the use of walking aids in the group but 57 patients ( 13.7 % ) improved , 38 of whom had undergone joint surgery .
	manualset3
171271	5	413227	7	NULL	NULL	0	NULL	group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There was an overall increase in disability ( Steinbrocker ) and the use of walking aids in the group but 57 patients ( 13.7 % ) improved , 38 of whom had undergone joint surgery .
	manualset3
171272	6	413227	7	NULL	NULL	0	NULL	57 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There was an overall increase in disability ( Steinbrocker ) and the use of walking aids in the group but 57 patients ( 13.7 % ) improved , 38 of whom had undergone joint surgery .
	manualset3
171273	7	413227	7	NULL	NULL	0	NULL	13.7 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was an overall increase in disability ( Steinbrocker ) and the use of walking aids in the group but 57 patients ( 13.7 % ) improved , 38 of whom had undergone joint surgery .
	manualset3
171274	8	413227	7	NULL	NULL	0	NULL	 38	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was an overall increase in disability ( Steinbrocker ) and the use of walking aids in the group but 57 patients ( 13.7 % ) improved , 38 of whom had undergone joint surgery .
	manualset3
171275	9	413227	7	NULL	NULL	0	NULL	joint surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There was an overall increase in disability ( Steinbrocker ) and the use of walking aids in the group but 57 patients ( 13.7 % ) improved , 38 of whom had undergone joint surgery .
	manualset3
171276	1	413228	7	NULL	NULL	0	NULL	tissue preservation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was good tissue preservation , due to a minimum delay between obtaining the specimens and fixation .
	manualset3
171277	2	413228	7	NULL	NULL	0	NULL	minimum delay	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	There was good tissue preservation , due to a minimum delay between obtaining the specimens and fixation .
	manualset3
171278	3	413228	7	NULL	NULL	0	NULL	specimens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	There was good tissue preservation , due to a minimum delay between obtaining the specimens and fixation .
	manualset3
171279	4	413228	7	NULL	NULL	0	NULL	fixation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There was good tissue preservation , due to a minimum delay between obtaining the specimens and fixation .
	manualset3
171280	1	413229	7	NULL	NULL	0	NULL	increased water excretion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was invariably increased water excretion when the ratio of urea to non-urea solute output exceeded 2.4 .
	manualset3
171281	2	413229	7	NULL	NULL	0	NULL	 ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was invariably increased water excretion when the ratio of urea to non-urea solute output exceeded 2.4 .
	manualset3
171282	3	413229	7	NULL	NULL	0	NULL	urea	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There was invariably increased water excretion when the ratio of urea to non-urea solute output exceeded 2.4 .
	manualset3
171283	4	413229	7	NULL	NULL	0	NULL	non-urea solute output	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was invariably increased water excretion when the ratio of urea to non-urea solute output exceeded 2.4 .
	manualset3
171284	5	413229	7	NULL	NULL	0	NULL	 2.4	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was invariably increased water excretion when the ratio of urea to non-urea solute output exceeded 2.4 .
	manualset3
171285	1	413230	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was little evidence of the latter and it was found that the digestibility of peas NSP ( 0.84 ) was considerably greater than that of wheat ( 0.65 ) .
	manualset3
171286	2	413230	7	NULL	NULL	0	NULL	digestibility 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was little evidence of the latter and it was found that the digestibility of peas NSP ( 0.84 ) was considerably greater than that of wheat ( 0.65 ) .
	manualset3
171287	3	413230	7	NULL	NULL	0	NULL	 peas NSP	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There was little evidence of the latter and it was found that the digestibility of peas NSP ( 0.84 ) was considerably greater than that of wheat ( 0.65 ) .
	manualset3
171288	4	413230	7	NULL	NULL	0	NULL	0.84	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was little evidence of the latter and it was found that the digestibility of peas NSP ( 0.84 ) was considerably greater than that of wheat ( 0.65 ) .
	manualset3
171289	5	413230	7	NULL	NULL	0	NULL	wheat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	There was little evidence of the latter and it was found that the digestibility of peas NSP ( 0.84 ) was considerably greater than that of wheat ( 0.65 ) .
	manualset3
171290	6	413230	7	NULL	NULL	0	NULL	 0.65	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was little evidence of the latter and it was found that the digestibility of peas NSP ( 0.84 ) was considerably greater than that of wheat ( 0.65 ) .
	manualset3
171340	1	413231	7	NULL	NULL	0	NULL	 IABP-related complication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no IABP-related complication in group I. IABP was very effective to perform OPCAB surgery safety .
	manualset3
171342	2	413231	7	NULL	NULL	0	NULL	group I	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no IABP-related complication in group I. IABP was very effective to perform OPCAB surgery safety .
	manualset3
171343	3	413231	7	NULL	NULL	0	NULL	IABP	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no IABP-related complication in group I. IABP was very effective to perform OPCAB surgery safety .
	manualset3
171344	4	413231	7	NULL	NULL	0	NULL	 OPCAB surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no IABP-related complication in group I. IABP was very effective to perform OPCAB surgery safety .
	manualset3
171345	1	413232	7	NULL	NULL	0	NULL	change	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no change in phospholipid contents .
	manualset3
171346	2	413232	7	NULL	NULL	0	NULL	phospholipid contents	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no change in phospholipid contents .
	manualset3
171347	1	413233	7	NULL	NULL	0	NULL	 change	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no change in the constitutive expression of Sox9 or bone morphogenetic protein 2 .
	manualset3
171348	2	413233	7	NULL	NULL	0	NULL	 constitutive expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no change in the constitutive expression of Sox9 or bone morphogenetic protein 2 .
	manualset3
171349	3	413233	7	NULL	NULL	0	NULL	Sox9	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no change in the constitutive expression of Sox9 or bone morphogenetic protein 2 .
	manualset3
171350	4	413233	7	NULL	NULL	0	NULL	bone morphogenetic protein 2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no change in the constitutive expression of Sox9 or bone morphogenetic protein 2 .
	manualset3
171351	1	413234	7	NULL	NULL	0	NULL	clear effect 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no clear effect of sex or nutrition on the assessment of the sensory attributes .
	manualset3
171352	2	413234	7	NULL	NULL	0	NULL	sex	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no clear effect of sex or nutrition on the assessment of the sensory attributes .
	manualset3
171353	3	413234	7	NULL	NULL	0	NULL	nutrition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no clear effect of sex or nutrition on the assessment of the sensory attributes .
	manualset3
171354	4	413234	7	NULL	NULL	0	NULL	 assessment	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no clear effect of sex or nutrition on the assessment of the sensory attributes .
	manualset3
171355	5	413234	7	NULL	NULL	0	NULL	sensory attributes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no clear effect of sex or nutrition on the assessment of the sensory attributes .
	manualset3
171356	1	413235	7	NULL	NULL	0	NULL	Activities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Activities in maritime medicine in countries of Central and Eastern Europe : symposia on maritime medicine , 1963-1989 .
	manualset3
171357	2	413235	7	NULL	NULL	0	NULL	maritime medicine	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Activities in maritime medicine in countries of Central and Eastern Europe : symposia on maritime medicine , 1963-1989 .
	manualset3
171358	3	413235	7	NULL	NULL	0	NULL	countries	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Activities in maritime medicine in countries of Central and Eastern Europe : symposia on maritime medicine , 1963-1989 .
	manualset3
171359	4	413235	7	NULL	NULL	0	NULL	 Central Europe	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Activities in maritime medicine in countries of Central and Eastern Europe : symposia on maritime medicine , 1963-1989 .
	manualset3
171360	5	413235	7	NULL	NULL	0	NULL	Eastern Europe	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Activities in maritime medicine in countries of Central and Eastern Europe : symposia on maritime medicine , 1963-1989 .
	manualset3
171361	6	413235	7	NULL	NULL	0	NULL	symposia 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Activities in maritime medicine in countries of Central and Eastern Europe : symposia on maritime medicine , 1963-1989 .
	manualset3
171362	7	413235	7	NULL	NULL	0	NULL	maritime medicine	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Activities in maritime medicine in countries of Central and Eastern Europe : symposia on maritime medicine , 1963-1989 .
	manualset3
171363	8	413235	7	NULL	NULL	0	NULL	1963-1989	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Activities in maritime medicine in countries of Central and Eastern Europe : symposia on maritime medicine , 1963-1989 .
	manualset3
171365	1	413236	7	NULL	NULL	0	NULL	no consistent pattern	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no consistent pattern of elevated odds ratios for glioma , meningioma , or acoustic neuroma with use or prolonged use of permanent , semipermanent , temporary , or gradual hair dyes .
	manualset3
171366	2	413236	7	NULL	NULL	0	NULL	elevated odds ratios	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no consistent pattern of elevated odds ratios for glioma , meningioma , or acoustic neuroma with use or prolonged use of permanent , semipermanent , temporary , or gradual hair dyes .
	manualset3
171367	3	413236	7	NULL	NULL	0	NULL	glioma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no consistent pattern of elevated odds ratios for glioma , meningioma , or acoustic neuroma with use or prolonged use of permanent , semipermanent , temporary , or gradual hair dyes .
	manualset3
171368	4	413236	7	NULL	NULL	0	NULL	meningioma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no consistent pattern of elevated odds ratios for glioma , meningioma , or acoustic neuroma with use or prolonged use of permanent , semipermanent , temporary , or gradual hair dyes .
	manualset3
171369	5	413236	7	NULL	NULL	0	NULL	acoustic neuroma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no consistent pattern of elevated odds ratios for glioma , meningioma , or acoustic neuroma with use or prolonged use of permanent , semipermanent , temporary , or gradual hair dyes .
	manualset3
171370	6	413236	7	NULL	NULL	0	NULL	use of permanent hair dyes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no consistent pattern of elevated odds ratios for glioma , meningioma , or acoustic neuroma with use or prolonged use of permanent , semipermanent , temporary , or gradual hair dyes .
	manualset3
171371	7	413236	7	NULL	NULL	0	NULL	use of semipermanent hair dyes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no consistent pattern of elevated odds ratios for glioma , meningioma , or acoustic neuroma with use or prolonged use of permanent , semipermanent , temporary , or gradual hair dyes .
	manualset3
171372	8	413236	7	NULL	NULL	0	NULL	use of temporary hair dyes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no consistent pattern of elevated odds ratios for glioma , meningioma , or acoustic neuroma with use or prolonged use of permanent , semipermanent , temporary , or gradual hair dyes .
	manualset3
171373	9	413236	7	NULL	NULL	0	NULL	use of gradual hair dyes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no consistent pattern of elevated odds ratios for glioma , meningioma , or acoustic neuroma with use or prolonged use of permanent , semipermanent , temporary , or gradual hair dyes .
	manualset3
171374	1	413237	7	NULL	NULL	0	NULL	no correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no correlation between elevated tumor markers and cytomegalovirus infection .
	manualset3
171375	2	413237	7	NULL	NULL	0	NULL	elevated tumor markers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no correlation between elevated tumor markers and cytomegalovirus infection .
	manualset3
171376	3	413237	7	NULL	NULL	0	NULL	cytomegalovirus infection	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no correlation between elevated tumor markers and cytomegalovirus infection .
	manualset3
171377	1	413238	7	NULL	NULL	0	NULL	no correlation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no correlation between injury rates and job experience .
	manualset3
171378	2	413238	7	NULL	NULL	0	NULL	 injury rates	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no correlation between injury rates and job experience .
	manualset3
171379	3	413238	7	NULL	NULL	0	NULL	 job experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no correlation between injury rates and job experience .
	manualset3
171380	1	413239	7	NULL	NULL	0	NULL	no correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no correlation between p53-overexpression in tissue and p53-protein levels in sera or between p53-autoantibody levels in sera , nor in mutation frequency of the p53-gene and p53-overexpression in tissue .
	manualset3
171381	2	413239	7	NULL	NULL	0	NULL	p53-overexpression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no correlation between p53-overexpression in tissue and p53-protein levels in sera or between p53-autoantibody levels in sera , nor in mutation frequency of the p53-gene and p53-overexpression in tissue .
	manualset3
171382	3	413239	7	NULL	NULL	0	NULL	tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no correlation between p53-overexpression in tissue and p53-protein levels in sera or between p53-autoantibody levels in sera , nor in mutation frequency of the p53-gene and p53-overexpression in tissue .
	manualset3
171383	4	413239	7	NULL	NULL	0	NULL	p53-protein levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no correlation between p53-overexpression in tissue and p53-protein levels in sera or between p53-autoantibody levels in sera , nor in mutation frequency of the p53-gene and p53-overexpression in tissue .
	manualset3
171384	5	413239	7	NULL	NULL	0	NULL	sera	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no correlation between p53-overexpression in tissue and p53-protein levels in sera or between p53-autoantibody levels in sera , nor in mutation frequency of the p53-gene and p53-overexpression in tissue .
	manualset3
171385	6	413239	7	NULL	NULL	0	NULL	p53-autoantibody levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no correlation between p53-overexpression in tissue and p53-protein levels in sera or between p53-autoantibody levels in sera , nor in mutation frequency of the p53-gene and p53-overexpression in tissue .
	manualset3
171386	7	413239	7	NULL	NULL	0	NULL	sera	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no correlation between p53-overexpression in tissue and p53-protein levels in sera or between p53-autoantibody levels in sera , nor in mutation frequency of the p53-gene and p53-overexpression in tissue .
	manualset3
171387	8	413239	7	NULL	NULL	0	NULL	mutation frequency 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no correlation between p53-overexpression in tissue and p53-protein levels in sera or between p53-autoantibody levels in sera , nor in mutation frequency of the p53-gene and p53-overexpression in tissue .
	manualset3
171388	9	413239	7	NULL	NULL	0	NULL	p53-gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no correlation between p53-overexpression in tissue and p53-protein levels in sera or between p53-autoantibody levels in sera , nor in mutation frequency of the p53-gene and p53-overexpression in tissue .
	manualset3
171389	10	413239	7	NULL	NULL	0	NULL	p53-overexpression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no correlation between p53-overexpression in tissue and p53-protein levels in sera or between p53-autoantibody levels in sera , nor in mutation frequency of the p53-gene and p53-overexpression in tissue .
	manualset3
171390	11	413239	7	NULL	NULL	0	NULL	 tissue 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no correlation between p53-overexpression in tissue and p53-protein levels in sera or between p53-autoantibody levels in sera , nor in mutation frequency of the p53-gene and p53-overexpression in tissue .
	manualset3
171391	1	413240	7	NULL	NULL	0	NULL	no difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no difference in renal eNOS and nNOS between allograft groups .
	manualset3
171392	2	413240	7	NULL	NULL	0	NULL	renal eNOS	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no difference in renal eNOS and nNOS between allograft groups .
	manualset3
171393	3	413240	7	NULL	NULL	0	NULL	nNOS	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no difference in renal eNOS and nNOS between allograft groups .
	manualset3
171394	4	413240	7	NULL	NULL	0	NULL	allograft groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no difference in renal eNOS and nNOS between allograft groups .
	manualset3
171395	1	413241	7	NULL	NULL	0	NULL	 no difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no difference in the Km of the Na + - H + antiporter among these five groups .
	manualset3
171396	2	413241	7	NULL	NULL	0	NULL	Km	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no difference in the Km of the Na + - H + antiporter among these five groups .
	manualset3
171397	3	413241	7	NULL	NULL	0	NULL	Na + - H + antiporter	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no difference in the Km of the Na + - H + antiporter among these five groups .
	manualset3
171398	4	413241	7	NULL	NULL	0	NULL	five groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no difference in the Km of the Na + - H + antiporter among these five groups .
	manualset3
171399	1	413242	7	NULL	NULL	0	NULL	no evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no evidence for a significant increase in the plant sterol content of the plasma of patients with hypercholesterolemia or hypertriglyceridemia .
	manualset3
171400	2	413242	7	NULL	NULL	0	NULL	 increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no evidence for a significant increase in the plant sterol content of the plasma of patients with hypercholesterolemia or hypertriglyceridemia .
	manualset3
171401	3	413242	7	NULL	NULL	0	NULL	plant sterol content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no evidence for a significant increase in the plant sterol content of the plasma of patients with hypercholesterolemia or hypertriglyceridemia .
	manualset3
171402	4	413242	7	NULL	NULL	0	NULL	 plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no evidence for a significant increase in the plant sterol content of the plasma of patients with hypercholesterolemia or hypertriglyceridemia .
	manualset3
171403	5	413242	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no evidence for a significant increase in the plant sterol content of the plasma of patients with hypercholesterolemia or hypertriglyceridemia .
	manualset3
171404	6	413242	7	NULL	NULL	0	NULL	hypercholesterolemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no evidence for a significant increase in the plant sterol content of the plasma of patients with hypercholesterolemia or hypertriglyceridemia .
	manualset3
171405	7	413242	7	NULL	NULL	0	NULL	 hypertriglyceridemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no evidence for a significant increase in the plant sterol content of the plasma of patients with hypercholesterolemia or hypertriglyceridemia .
	manualset3
171406	1	413243	7	NULL	NULL	0	NULL	no evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no evidence of differentiation into B cells .
	manualset3
171407	2	413243	7	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no evidence of differentiation into B cells .
	manualset3
171408	3	413243	7	NULL	NULL	0	NULL	 B cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no evidence of differentiation into B cells .
	manualset3
171409	1	413244	7	NULL	NULL	0	NULL	Activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activities of monoamine oxidase B , Cu-Zn-dependent superoxide dismutase ( SOD ) , and catalase , the concentration of enzyme-active ceruloplasmin , and resistance of the nerve tissue to oxidative stress were examined in spinal cord preparations from humans ( n = 43 ) died at the age of 21-92 years .
	manualset3
171410	2	413244	7	NULL	NULL	0	NULL	monoamine oxidase B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Activities of monoamine oxidase B , Cu-Zn-dependent superoxide dismutase ( SOD ) , and catalase , the concentration of enzyme-active ceruloplasmin , and resistance of the nerve tissue to oxidative stress were examined in spinal cord preparations from humans ( n = 43 ) died at the age of 21-92 years .
	manualset3
171411	3	413244	7	NULL	NULL	0	NULL	Cu-Zn-dependent superoxide dismutase ( SOD )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Activities of monoamine oxidase B , Cu-Zn-dependent superoxide dismutase ( SOD ) , and catalase , the concentration of enzyme-active ceruloplasmin , and resistance of the nerve tissue to oxidative stress were examined in spinal cord preparations from humans ( n = 43 ) died at the age of 21-92 years .
	manualset3
171412	4	413244	7	NULL	NULL	0	NULL	catalase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Activities of monoamine oxidase B , Cu-Zn-dependent superoxide dismutase ( SOD ) , and catalase , the concentration of enzyme-active ceruloplasmin , and resistance of the nerve tissue to oxidative stress were examined in spinal cord preparations from humans ( n = 43 ) died at the age of 21-92 years .
	manualset3
171413	5	413244	7	NULL	NULL	0	NULL	concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Activities of monoamine oxidase B , Cu-Zn-dependent superoxide dismutase ( SOD ) , and catalase , the concentration of enzyme-active ceruloplasmin , and resistance of the nerve tissue to oxidative stress were examined in spinal cord preparations from humans ( n = 43 ) died at the age of 21-92 years .
	manualset3
171414	6	413244	7	NULL	NULL	0	NULL	enzyme-active ceruloplasmin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Activities of monoamine oxidase B , Cu-Zn-dependent superoxide dismutase ( SOD ) , and catalase , the concentration of enzyme-active ceruloplasmin , and resistance of the nerve tissue to oxidative stress were examined in spinal cord preparations from humans ( n = 43 ) died at the age of 21-92 years .
	manualset3
171415	7	413244	7	NULL	NULL	0	NULL	resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activities of monoamine oxidase B , Cu-Zn-dependent superoxide dismutase ( SOD ) , and catalase , the concentration of enzyme-active ceruloplasmin , and resistance of the nerve tissue to oxidative stress were examined in spinal cord preparations from humans ( n = 43 ) died at the age of 21-92 years .
	manualset3
171416	8	413244	7	NULL	NULL	0	NULL	nerve tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Activities of monoamine oxidase B , Cu-Zn-dependent superoxide dismutase ( SOD ) , and catalase , the concentration of enzyme-active ceruloplasmin , and resistance of the nerve tissue to oxidative stress were examined in spinal cord preparations from humans ( n = 43 ) died at the age of 21-92 years .
	manualset3
171417	9	413244	7	NULL	NULL	0	NULL	oxidative stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Activities of monoamine oxidase B , Cu-Zn-dependent superoxide dismutase ( SOD ) , and catalase , the concentration of enzyme-active ceruloplasmin , and resistance of the nerve tissue to oxidative stress were examined in spinal cord preparations from humans ( n = 43 ) died at the age of 21-92 years .
	manualset3
171418	10	413244	7	NULL	NULL	0	NULL	 spinal cord preparations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Activities of monoamine oxidase B , Cu-Zn-dependent superoxide dismutase ( SOD ) , and catalase , the concentration of enzyme-active ceruloplasmin , and resistance of the nerve tissue to oxidative stress were examined in spinal cord preparations from humans ( n = 43 ) died at the age of 21-92 years .
	manualset3
171419	11	413244	7	NULL	NULL	0	NULL	 humans 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Activities of monoamine oxidase B , Cu-Zn-dependent superoxide dismutase ( SOD ) , and catalase , the concentration of enzyme-active ceruloplasmin , and resistance of the nerve tissue to oxidative stress were examined in spinal cord preparations from humans ( n = 43 ) died at the age of 21-92 years .
	manualset3
171420	12	413244	7	NULL	NULL	0	NULL	n = 43	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Activities of monoamine oxidase B , Cu-Zn-dependent superoxide dismutase ( SOD ) , and catalase , the concentration of enzyme-active ceruloplasmin , and resistance of the nerve tissue to oxidative stress were examined in spinal cord preparations from humans ( n = 43 ) died at the age of 21-92 years .
	manualset3
171421	13	413244	7	NULL	NULL	0	NULL	age	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Activities of monoamine oxidase B , Cu-Zn-dependent superoxide dismutase ( SOD ) , and catalase , the concentration of enzyme-active ceruloplasmin , and resistance of the nerve tissue to oxidative stress were examined in spinal cord preparations from humans ( n = 43 ) died at the age of 21-92 years .
	manualset3
171422	14	413244	7	NULL	NULL	0	NULL	21-92 years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Activities of monoamine oxidase B , Cu-Zn-dependent superoxide dismutase ( SOD ) , and catalase , the concentration of enzyme-active ceruloplasmin , and resistance of the nerve tissue to oxidative stress were examined in spinal cord preparations from humans ( n = 43 ) died at the age of 21-92 years .
	manualset3
171423	1	413245	7	NULL	NULL	NULL	NULL	no incorporation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There was no incorporation of IPP into cis-1 , 4 - polyisoprene in the absence of rubber particles as primer , and Langmuir isotherm plots showed that the specific activity of the enzyme was proportional to the concentration of the enzyme on the surface of the rubber particles .
	manualset3
171424	2	413245	7	NULL	NULL	0	NULL	IPP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no incorporation of IPP into cis-1 , 4 - polyisoprene in the absence of rubber particles as primer , and Langmuir isotherm plots showed that the specific activity of the enzyme was proportional to the concentration of the enzyme on the surface of the rubber particles .
	manualset3
171425	3	413245	7	NULL	NULL	0	NULL	cis-1 , 4 - polyisoprene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no incorporation of IPP into cis-1 , 4 - polyisoprene in the absence of rubber particles as primer , and Langmuir isotherm plots showed that the specific activity of the enzyme was proportional to the concentration of the enzyme on the surface of the rubber particles .
	manualset3
171426	4	413245	7	NULL	NULL	0	NULL	absence 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no incorporation of IPP into cis-1 , 4 - polyisoprene in the absence of rubber particles as primer , and Langmuir isotherm plots showed that the specific activity of the enzyme was proportional to the concentration of the enzyme on the surface of the rubber particles .
	manualset3
171427	5	413245	7	NULL	NULL	0	NULL	rubber particles	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no incorporation of IPP into cis-1 , 4 - polyisoprene in the absence of rubber particles as primer , and Langmuir isotherm plots showed that the specific activity of the enzyme was proportional to the concentration of the enzyme on the surface of the rubber particles .
	manualset3
171428	6	413245	7	NULL	NULL	0	NULL	primer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no incorporation of IPP into cis-1 , 4 - polyisoprene in the absence of rubber particles as primer , and Langmuir isotherm plots showed that the specific activity of the enzyme was proportional to the concentration of the enzyme on the surface of the rubber particles .
	manualset3
171429	7	413245	7	NULL	NULL	0	NULL	Langmuir isotherm plots	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no incorporation of IPP into cis-1 , 4 - polyisoprene in the absence of rubber particles as primer , and Langmuir isotherm plots showed that the specific activity of the enzyme was proportional to the concentration of the enzyme on the surface of the rubber particles .
	manualset3
171430	8	413245	7	NULL	NULL	0	NULL	 specific activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no incorporation of IPP into cis-1 , 4 - polyisoprene in the absence of rubber particles as primer , and Langmuir isotherm plots showed that the specific activity of the enzyme was proportional to the concentration of the enzyme on the surface of the rubber particles .
	manualset3
171431	9	413245	7	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no incorporation of IPP into cis-1 , 4 - polyisoprene in the absence of rubber particles as primer , and Langmuir isotherm plots showed that the specific activity of the enzyme was proportional to the concentration of the enzyme on the surface of the rubber particles .
	manualset3
171432	10	413245	7	NULL	NULL	0	NULL	concentration of the enzyme	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no incorporation of IPP into cis-1 , 4 - polyisoprene in the absence of rubber particles as primer , and Langmuir isotherm plots showed that the specific activity of the enzyme was proportional to the concentration of the enzyme on the surface of the rubber particles .
	manualset3
171433	11	413245	7	NULL	NULL	0	NULL	 surface of the rubber particles	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no incorporation of IPP into cis-1 , 4 - polyisoprene in the absence of rubber particles as primer , and Langmuir isotherm plots showed that the specific activity of the enzyme was proportional to the concentration of the enzyme on the surface of the rubber particles .
	manualset3
171434	1	413246	7	NULL	NULL	0	NULL	no modification	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no modification of contraction time and time of half relaxation ( T 1/2R ) .
	manualset3
171435	2	413246	7	NULL	NULL	0	NULL	contraction time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no modification of contraction time and time of half relaxation ( T 1/2R ) .
	manualset3
171436	3	413246	7	NULL	NULL	0	NULL	time of half relaxation ( T 1/2R )	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no modification of contraction time and time of half relaxation ( T 1/2R ) .
	manualset3
171437	1	413247	7	NULL	NULL	0	NULL	no reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no reaction with rHDL and LDL , but 30 % of the activity with PNPB was retained .
	manualset3
171438	2	413247	7	NULL	NULL	0	NULL	rHDL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no reaction with rHDL and LDL , but 30 % of the activity with PNPB was retained .
	manualset3
171439	3	413247	7	NULL	NULL	0	NULL	LDL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no reaction with rHDL and LDL , but 30 % of the activity with PNPB was retained .
	manualset3
171440	4	413247	7	NULL	NULL	0	NULL	 30 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no reaction with rHDL and LDL , but 30 % of the activity with PNPB was retained .
	manualset3
171441	5	413247	7	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no reaction with rHDL and LDL , but 30 % of the activity with PNPB was retained .
	manualset3
171442	6	413247	7	NULL	NULL	0	NULL	PNPB	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no reaction with rHDL and LDL , but 30 % of the activity with PNPB was retained .
	manualset3
171443	1	413248	7	NULL	NULL	0	NULL	no relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no relationship between lytic ability and Gm allotype or D epitope specificity of the antibodies .
	manualset3
171444	2	413248	7	NULL	NULL	0	NULL	lytic ability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no relationship between lytic ability and Gm allotype or D epitope specificity of the antibodies .
	manualset3
171445	3	413248	7	NULL	NULL	0	NULL	Gm allotype	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no relationship between lytic ability and Gm allotype or D epitope specificity of the antibodies .
	manualset3
171446	4	413248	7	NULL	NULL	NULL	NULL	 D epitope specificity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There was no relationship between lytic ability and Gm allotype or D epitope specificity of the antibodies .
	manualset3
171447	5	413248	7	NULL	NULL	0	NULL	antibodies	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no relationship between lytic ability and Gm allotype or D epitope specificity of the antibodies .
	manualset3
171448	1	413249	7	NULL	NULL	0	NULL	no significant difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between patients with receptor-positive and receptor-negative tumors in the relapse-free interval , but survival from first relapse was longer in patients with receptor-positive tumors .
	manualset3
171449	2	413249	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between patients with receptor-positive and receptor-negative tumors in the relapse-free interval , but survival from first relapse was longer in patients with receptor-positive tumors .
	manualset3
171450	3	413249	7	NULL	NULL	0	NULL	 receptor-positive tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between patients with receptor-positive and receptor-negative tumors in the relapse-free interval , but survival from first relapse was longer in patients with receptor-positive tumors .
	manualset3
171451	4	413249	7	NULL	NULL	0	NULL	receptor-negative tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between patients with receptor-positive and receptor-negative tumors in the relapse-free interval , but survival from first relapse was longer in patients with receptor-positive tumors .
	manualset3
171452	5	413249	7	NULL	NULL	0	NULL	 relapse-free interval	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between patients with receptor-positive and receptor-negative tumors in the relapse-free interval , but survival from first relapse was longer in patients with receptor-positive tumors .
	manualset3
171453	6	413249	7	NULL	NULL	0	NULL	survival 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between patients with receptor-positive and receptor-negative tumors in the relapse-free interval , but survival from first relapse was longer in patients with receptor-positive tumors .
	manualset3
171454	7	413249	7	NULL	NULL	NULL	NULL	first relapse	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There was no significant difference between patients with receptor-positive and receptor-negative tumors in the relapse-free interval , but survival from first relapse was longer in patients with receptor-positive tumors .
	manualset3
171455	8	413249	7	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between patients with receptor-positive and receptor-negative tumors in the relapse-free interval , but survival from first relapse was longer in patients with receptor-positive tumors .
	manualset3
171456	9	413249	7	NULL	NULL	0	NULL	receptor-positive tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between patients with receptor-positive and receptor-negative tumors in the relapse-free interval , but survival from first relapse was longer in patients with receptor-positive tumors .
	manualset3
171457	1	413250	7	NULL	NULL	0	NULL	no significant difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between poultry and human C. jejuni strains concerning the transcription levels of cmeABC and Cj0561c in cultures without bile salts and concerning bile-salt-induced changes in transcription of cmeABC and Cj0561c .
	manualset3
171458	2	413250	7	NULL	NULL	0	NULL	poultry C. jejuni strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between poultry and human C. jejuni strains concerning the transcription levels of cmeABC and Cj0561c in cultures without bile salts and concerning bile-salt-induced changes in transcription of cmeABC and Cj0561c .
	manualset3
171459	3	413250	7	NULL	NULL	0	NULL	 human C. jejuni strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between poultry and human C. jejuni strains concerning the transcription levels of cmeABC and Cj0561c in cultures without bile salts and concerning bile-salt-induced changes in transcription of cmeABC and Cj0561c .
	manualset3
171460	4	413250	7	NULL	NULL	0	NULL	transcription levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between poultry and human C. jejuni strains concerning the transcription levels of cmeABC and Cj0561c in cultures without bile salts and concerning bile-salt-induced changes in transcription of cmeABC and Cj0561c .
	manualset3
171461	5	413250	7	NULL	NULL	0	NULL	cmeABC 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between poultry and human C. jejuni strains concerning the transcription levels of cmeABC and Cj0561c in cultures without bile salts and concerning bile-salt-induced changes in transcription of cmeABC and Cj0561c .
	manualset3
171462	6	413250	7	NULL	NULL	0	NULL	Cj0561c	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between poultry and human C. jejuni strains concerning the transcription levels of cmeABC and Cj0561c in cultures without bile salts and concerning bile-salt-induced changes in transcription of cmeABC and Cj0561c .
	manualset3
171463	7	413250	7	NULL	NULL	0	NULL	cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between poultry and human C. jejuni strains concerning the transcription levels of cmeABC and Cj0561c in cultures without bile salts and concerning bile-salt-induced changes in transcription of cmeABC and Cj0561c .
	manualset3
171464	8	413250	7	NULL	NULL	0	NULL	bile salts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between poultry and human C. jejuni strains concerning the transcription levels of cmeABC and Cj0561c in cultures without bile salts and concerning bile-salt-induced changes in transcription of cmeABC and Cj0561c .
	manualset3
171465	9	413250	7	NULL	NULL	0	NULL	bile-salt-induced changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between poultry and human C. jejuni strains concerning the transcription levels of cmeABC and Cj0561c in cultures without bile salts and concerning bile-salt-induced changes in transcription of cmeABC and Cj0561c .
	manualset3
171466	10	413250	7	NULL	NULL	0	NULL	transcription 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between poultry and human C. jejuni strains concerning the transcription levels of cmeABC and Cj0561c in cultures without bile salts and concerning bile-salt-induced changes in transcription of cmeABC and Cj0561c .
	manualset3
171467	11	413250	7	NULL	NULL	0	NULL	cmeABC	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between poultry and human C. jejuni strains concerning the transcription levels of cmeABC and Cj0561c in cultures without bile salts and concerning bile-salt-induced changes in transcription of cmeABC and Cj0561c .
	manualset3
171468	12	413250	7	NULL	NULL	0	NULL	 Cj0561c	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between poultry and human C. jejuni strains concerning the transcription levels of cmeABC and Cj0561c in cultures without bile salts and concerning bile-salt-induced changes in transcription of cmeABC and Cj0561c .
	manualset3
171469	1	413251	7	NULL	NULL	0	NULL	no significant difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between the two arms of the gastric or pancreatic adenocarcinoma groups , with a median survival of 13 months and 11.5 months respectively in gastric carcinoma , and 7.8 months and 7.3 months in pancreatic carcinoma .
	manualset3
171470	2	413251	7	NULL	NULL	0	NULL	 two arms	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between the two arms of the gastric or pancreatic adenocarcinoma groups , with a median survival of 13 months and 11.5 months respectively in gastric carcinoma , and 7.8 months and 7.3 months in pancreatic carcinoma .
	manualset3
171471	3	413251	7	NULL	NULL	0	NULL	gastric adenocarcinoma groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between the two arms of the gastric or pancreatic adenocarcinoma groups , with a median survival of 13 months and 11.5 months respectively in gastric carcinoma , and 7.8 months and 7.3 months in pancreatic carcinoma .
	manualset3
171472	4	413251	7	NULL	NULL	0	NULL	pancreatic adenocarcinoma groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between the two arms of the gastric or pancreatic adenocarcinoma groups , with a median survival of 13 months and 11.5 months respectively in gastric carcinoma , and 7.8 months and 7.3 months in pancreatic carcinoma .
	manualset3
171473	5	413251	7	NULL	NULL	0	NULL	median survival	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between the two arms of the gastric or pancreatic adenocarcinoma groups , with a median survival of 13 months and 11.5 months respectively in gastric carcinoma , and 7.8 months and 7.3 months in pancreatic carcinoma .
	manualset3
171474	6	413251	7	NULL	NULL	0	NULL	13 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between the two arms of the gastric or pancreatic adenocarcinoma groups , with a median survival of 13 months and 11.5 months respectively in gastric carcinoma , and 7.8 months and 7.3 months in pancreatic carcinoma .
	manualset3
171475	7	413251	7	NULL	NULL	0	NULL	11.5 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between the two arms of the gastric or pancreatic adenocarcinoma groups , with a median survival of 13 months and 11.5 months respectively in gastric carcinoma , and 7.8 months and 7.3 months in pancreatic carcinoma .
	manualset3
171476	8	413251	7	NULL	NULL	0	NULL	gastric carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between the two arms of the gastric or pancreatic adenocarcinoma groups , with a median survival of 13 months and 11.5 months respectively in gastric carcinoma , and 7.8 months and 7.3 months in pancreatic carcinoma .
	manualset3
171477	9	413251	7	NULL	NULL	0	NULL	 7.8 months 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between the two arms of the gastric or pancreatic adenocarcinoma groups , with a median survival of 13 months and 11.5 months respectively in gastric carcinoma , and 7.8 months and 7.3 months in pancreatic carcinoma .
	manualset3
171478	10	413251	7	NULL	NULL	0	NULL	7.3 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between the two arms of the gastric or pancreatic adenocarcinoma groups , with a median survival of 13 months and 11.5 months respectively in gastric carcinoma , and 7.8 months and 7.3 months in pancreatic carcinoma .
	manualset3
171479	11	413251	7	NULL	NULL	0	NULL	 pancreatic carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference between the two arms of the gastric or pancreatic adenocarcinoma groups , with a median survival of 13 months and 11.5 months respectively in gastric carcinoma , and 7.8 months and 7.3 months in pancreatic carcinoma .
	manualset3
171480	1	413252	7	NULL	NULL	0	NULL	no significant difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference in test performance between students who preferred visual and reading/writing learning styles ( self-reported and assessed ) .
	manualset3
171481	2	413252	7	NULL	NULL	0	NULL	test performance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference in test performance between students who preferred visual and reading/writing learning styles ( self-reported and assessed ) .
	manualset3
171482	3	413252	7	NULL	NULL	0	NULL	students	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference in test performance between students who preferred visual and reading/writing learning styles ( self-reported and assessed ) .
	manualset3
171483	4	413252	7	NULL	NULL	0	NULL	 visual learning styles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference in test performance between students who preferred visual and reading/writing learning styles ( self-reported and assessed ) .
	manualset3
171484	5	413252	7	NULL	NULL	0	NULL	reading/writing learning styles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference in test performance between students who preferred visual and reading/writing learning styles ( self-reported and assessed ) .
	manualset3
171485	1	413253	7	NULL	NULL	0	NULL	Activities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activities were similar in men and women .
	manualset3
171486	2	413253	7	NULL	NULL	0	NULL	 similar	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Activities were similar in men and women .
	manualset3
171487	3	413253	7	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Activities were similar in men and women .
	manualset3
171488	4	413253	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Activities were similar in men and women .
	manualset3
171489	1	413254	7	NULL	NULL	0	NULL	no significant difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference in the level of apoptosis induced between these controls and cultures not exposed to cerebrospinal fluid at all .
	manualset3
171490	2	413254	7	NULL	NULL	0	NULL	level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference in the level of apoptosis induced between these controls and cultures not exposed to cerebrospinal fluid at all .
	manualset3
171491	3	413254	7	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference in the level of apoptosis induced between these controls and cultures not exposed to cerebrospinal fluid at all .
	manualset3
171492	4	413254	7	NULL	NULL	0	NULL	 controls	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference in the level of apoptosis induced between these controls and cultures not exposed to cerebrospinal fluid at all .
	manualset3
171493	5	413254	7	NULL	NULL	0	NULL	cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference in the level of apoptosis induced between these controls and cultures not exposed to cerebrospinal fluid at all .
	manualset3
171494	6	413254	7	NULL	NULL	0	NULL	cerebrospinal fluid	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference in the level of apoptosis induced between these controls and cultures not exposed to cerebrospinal fluid at all .
	manualset3
171495	1	413255	7	NULL	NULL	0	NULL	no significant difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference in the presence of live virus or viral DNA in the nasal secretions or PBMCs between the two groups .
	manualset3
171496	2	413255	7	NULL	NULL	NULL	NULL	presence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There was no significant difference in the presence of live virus or viral DNA in the nasal secretions or PBMCs between the two groups .
	manualset3
171497	3	413255	7	NULL	NULL	0	NULL	live virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference in the presence of live virus or viral DNA in the nasal secretions or PBMCs between the two groups .
	manualset3
171498	4	413255	7	NULL	NULL	0	NULL	viral DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference in the presence of live virus or viral DNA in the nasal secretions or PBMCs between the two groups .
	manualset3
171499	5	413255	7	NULL	NULL	0	NULL	nasal secretions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference in the presence of live virus or viral DNA in the nasal secretions or PBMCs between the two groups .
	manualset3
171500	6	413255	7	NULL	NULL	0	NULL	PBMCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference in the presence of live virus or viral DNA in the nasal secretions or PBMCs between the two groups .
	manualset3
171501	7	413255	7	NULL	NULL	0	NULL	two groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference in the presence of live virus or viral DNA in the nasal secretions or PBMCs between the two groups .
	manualset3
171502	1	413256	7	NULL	NULL	0	NULL	no significant difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference in the prevalence of all three mutations between individuals affected with CVD or other forms of thromboembolic disease and healthy individuals .
	manualset3
171503	2	413256	7	NULL	NULL	0	NULL	prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference in the prevalence of all three mutations between individuals affected with CVD or other forms of thromboembolic disease and healthy individuals .
	manualset3
171504	3	413256	7	NULL	NULL	0	NULL	 three mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference in the prevalence of all three mutations between individuals affected with CVD or other forms of thromboembolic disease and healthy individuals .
	manualset3
171505	4	413256	7	NULL	NULL	0	NULL	 individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference in the prevalence of all three mutations between individuals affected with CVD or other forms of thromboembolic disease and healthy individuals .
	manualset3
171506	5	413256	7	NULL	NULL	0	NULL	CVD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference in the prevalence of all three mutations between individuals affected with CVD or other forms of thromboembolic disease and healthy individuals .
	manualset3
171507	6	413256	7	NULL	NULL	0	NULL	 forms of thromboembolic disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference in the prevalence of all three mutations between individuals affected with CVD or other forms of thromboembolic disease and healthy individuals .
	manualset3
171508	7	413256	7	NULL	NULL	0	NULL	healthy individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant difference in the prevalence of all three mutations between individuals affected with CVD or other forms of thromboembolic disease and healthy individuals .
	manualset3
171509	1	413257	7	NULL	NULL	0	NULL	no significant influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant influence of the atrial blanking time onto the measured parameters ( least square means + / - standard error ) with VAF between 281 + / - 12 and 300 + / - 12 ms ( P = NS ) , AFs between 3.4 + / - 0.2 and 3.6 + / - 0.2 beats ( P = NS ) and XAF between 1.84 + / - 0.12 and 2.03 + / - 0.12 beats ( P = NS ) .
	manualset3
171510	2	413257	7	NULL	NULL	0	NULL	atrial blanking time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant influence of the atrial blanking time onto the measured parameters ( least square means + / - standard error ) with VAF between 281 + / - 12 and 300 + / - 12 ms ( P = NS ) , AFs between 3.4 + / - 0.2 and 3.6 + / - 0.2 beats ( P = NS ) and XAF between 1.84 + / - 0.12 and 2.03 + / - 0.12 beats ( P = NS ) .
	manualset3
171511	3	413257	7	NULL	NULL	0	NULL	measured parameters 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant influence of the atrial blanking time onto the measured parameters ( least square means + / - standard error ) with VAF between 281 + / - 12 and 300 + / - 12 ms ( P = NS ) , AFs between 3.4 + / - 0.2 and 3.6 + / - 0.2 beats ( P = NS ) and XAF between 1.84 + / - 0.12 and 2.03 + / - 0.12 beats ( P = NS ) .
	manualset3
171512	4	413257	7	NULL	NULL	0	NULL	 least square means + / - standard error	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant influence of the atrial blanking time onto the measured parameters ( least square means + / - standard error ) with VAF between 281 + / - 12 and 300 + / - 12 ms ( P = NS ) , AFs between 3.4 + / - 0.2 and 3.6 + / - 0.2 beats ( P = NS ) and XAF between 1.84 + / - 0.12 and 2.03 + / - 0.12 beats ( P = NS ) .
	manualset3
171513	5	413257	7	NULL	NULL	0	NULL	VAF	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant influence of the atrial blanking time onto the measured parameters ( least square means + / - standard error ) with VAF between 281 + / - 12 and 300 + / - 12 ms ( P = NS ) , AFs between 3.4 + / - 0.2 and 3.6 + / - 0.2 beats ( P = NS ) and XAF between 1.84 + / - 0.12 and 2.03 + / - 0.12 beats ( P = NS ) .
	manualset3
171514	6	413257	7	NULL	NULL	0	NULL	 281 + / - 12	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant influence of the atrial blanking time onto the measured parameters ( least square means + / - standard error ) with VAF between 281 + / - 12 and 300 + / - 12 ms ( P = NS ) , AFs between 3.4 + / - 0.2 and 3.6 + / - 0.2 beats ( P = NS ) and XAF between 1.84 + / - 0.12 and 2.03 + / - 0.12 beats ( P = NS ) .
	manualset3
171515	7	413257	7	NULL	NULL	0	NULL	300 + / - 12 ms ( P = NS )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant influence of the atrial blanking time onto the measured parameters ( least square means + / - standard error ) with VAF between 281 + / - 12 and 300 + / - 12 ms ( P = NS ) , AFs between 3.4 + / - 0.2 and 3.6 + / - 0.2 beats ( P = NS ) and XAF between 1.84 + / - 0.12 and 2.03 + / - 0.12 beats ( P = NS ) .
	manualset3
171516	8	413257	7	NULL	NULL	NULL	NULL	AFs between 3.4 + / - 0.2 and 3.6 + / - 0.2 beats ( P = NS )	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There was no significant influence of the atrial blanking time onto the measured parameters ( least square means + / - standard error ) with VAF between 281 + / - 12 and 300 + / - 12 ms ( P = NS ) , AFs between 3.4 + / - 0.2 and 3.6 + / - 0.2 beats ( P = NS ) and XAF between 1.84 + / - 0.12 and 2.03 + / - 0.12 beats ( P = NS ) .
	manualset3
171517	9	413257	7	NULL	NULL	0	NULL	XAF between 1.84 + / - 0.12 and 2.03 + / - 0.12 beats ( P = NS )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no significant influence of the atrial blanking time onto the measured parameters ( least square means + / - standard error ) with VAF between 281 + / - 12 and 300 + / - 12 ms ( P = NS ) , AFs between 3.4 + / - 0.2 and 3.6 + / - 0.2 beats ( P = NS ) and XAF between 1.84 + / - 0.12 and 2.03 + / - 0.12 beats ( P = NS ) .
	manualset3
171518	1	413258	7	NULL	NULL	0	NULL	no statistically significant difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no statistically significant difference between patients with visceral metastasis ( 44.0 + / -16.8 ng/ml ) and patients with bone metastasis ( 35.2 + / -15.0 ng/ml ) ( p ) 0.05 ) .
	manualset3
171519	2	413258	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no statistically significant difference between patients with visceral metastasis ( 44.0 + / -16.8 ng/ml ) and patients with bone metastasis ( 35.2 + / -15.0 ng/ml ) ( p ) 0.05 ) .
	manualset3
171520	3	413258	7	NULL	NULL	0	NULL	visceral metastasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no statistically significant difference between patients with visceral metastasis ( 44.0 + / -16.8 ng/ml ) and patients with bone metastasis ( 35.2 + / -15.0 ng/ml ) ( p ) 0.05 ) .
	manualset3
171521	4	413258	7	NULL	NULL	NULL	NULL	44.0 + / -16.8 ng/ml	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There was no statistically significant difference between patients with visceral metastasis ( 44.0 + / -16.8 ng/ml ) and patients with bone metastasis ( 35.2 + / -15.0 ng/ml ) ( p ) 0.05 ) .
	manualset3
171522	5	413258	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no statistically significant difference between patients with visceral metastasis ( 44.0 + / -16.8 ng/ml ) and patients with bone metastasis ( 35.2 + / -15.0 ng/ml ) ( p ) 0.05 ) .
	manualset3
171523	6	413258	7	NULL	NULL	0	NULL	bone metastasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no statistically significant difference between patients with visceral metastasis ( 44.0 + / -16.8 ng/ml ) and patients with bone metastasis ( 35.2 + / -15.0 ng/ml ) ( p ) 0.05 ) .
	manualset3
171524	7	413258	7	NULL	NULL	0	NULL	 35.2 + / -15.0 ng/ml ) ( p ) 0.05	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no statistically significant difference between patients with visceral metastasis ( 44.0 + / -16.8 ng/ml ) and patients with bone metastasis ( 35.2 + / -15.0 ng/ml ) ( p ) 0.05 ) .
	manualset3
171525	1	413259	7	NULL	NULL	0	NULL	treatment-related effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no treatment-related effect on seminal vesicle or prostate weights .
	manualset3
171526	2	413259	7	NULL	NULL	0	NULL	seminal vesicle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no treatment-related effect on seminal vesicle or prostate weights .
	manualset3
171527	3	413259	7	NULL	NULL	0	NULL	prostate weights	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no treatment-related effect on seminal vesicle or prostate weights .
	manualset3
171528	1	413260	7	NULL	NULL	0	NULL	one exception	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There was one exception in which all the clones examined had inactive vif , suggesting a probable association of inactive vif with the nonprogression .
	manualset3
171529	2	413260	7	NULL	NULL	0	NULL	clones 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	There was one exception in which all the clones examined had inactive vif , suggesting a probable association of inactive vif with the nonprogression .
	manualset3
171530	3	413260	7	NULL	NULL	0	NULL	inactive vif	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	There was one exception in which all the clones examined had inactive vif , suggesting a probable association of inactive vif with the nonprogression .
	manualset3
171531	4	413260	7	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was one exception in which all the clones examined had inactive vif , suggesting a probable association of inactive vif with the nonprogression .
	manualset3
171532	5	413260	7	NULL	NULL	0	NULL	inactive vif 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	There was one exception in which all the clones examined had inactive vif , suggesting a probable association of inactive vif with the nonprogression .
	manualset3
171533	6	413260	7	NULL	NULL	0	NULL	nonprogression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was one exception in which all the clones examined had inactive vif , suggesting a probable association of inactive vif with the nonprogression .
	manualset3
171534	1	413261	7	NULL	NULL	0	NULL	Activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity in the left frontal region was more significant than that in other areas during beat imagination .
	manualset3
171535	2	413261	7	NULL	NULL	0	NULL	left frontal region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity in the left frontal region was more significant than that in other areas during beat imagination .
	manualset3
171536	3	413261	7	NULL	NULL	0	NULL	 areas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity in the left frontal region was more significant than that in other areas during beat imagination .
	manualset3
171537	4	413261	7	NULL	NULL	0	NULL	beat imagination	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity in the left frontal region was more significant than that in other areas during beat imagination .
	manualset3
171538	1	413262	7	NULL	NULL	0	NULL	substantial clinical overlap	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was substantial clinical overlap between pneumonia and malaria ( n = 895 ) , and between malaria and malnutrition ( n = 811 ) .
	manualset3
171539	2	413262	7	NULL	NULL	0	NULL	 pneumonia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There was substantial clinical overlap between pneumonia and malaria ( n = 895 ) , and between malaria and malnutrition ( n = 811 ) .
	manualset3
171540	3	413262	7	NULL	NULL	0	NULL	malaria	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There was substantial clinical overlap between pneumonia and malaria ( n = 895 ) , and between malaria and malnutrition ( n = 811 ) .
	manualset3
171541	4	413262	7	NULL	NULL	0	NULL	n = 895	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was substantial clinical overlap between pneumonia and malaria ( n = 895 ) , and between malaria and malnutrition ( n = 811 ) .
	manualset3
171542	5	413262	7	NULL	NULL	0	NULL	malaria	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There was substantial clinical overlap between pneumonia and malaria ( n = 895 ) , and between malaria and malnutrition ( n = 811 ) .
	manualset3
171543	6	413262	7	NULL	NULL	0	NULL	malnutrition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was substantial clinical overlap between pneumonia and malaria ( n = 895 ) , and between malaria and malnutrition ( n = 811 ) .
	manualset3
171544	7	413262	7	NULL	NULL	0	NULL	n = 811	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There was substantial clinical overlap between pneumonia and malaria ( n = 895 ) , and between malaria and malnutrition ( n = 811 ) .
	manualset3
171545	1	413263	7	NULL	NULL	0	NULL	synchronism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was synchronism in changing of LPO and neutrophilic phagocytic activity .
	manualset3
171546	2	413263	7	NULL	NULL	0	NULL	changing	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was synchronism in changing of LPO and neutrophilic phagocytic activity .
	manualset3
171547	3	413263	7	NULL	NULL	0	NULL	LPO	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was synchronism in changing of LPO and neutrophilic phagocytic activity .
	manualset3
171548	4	413263	7	NULL	NULL	0	NULL	neutrophilic phagocytic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was synchronism in changing of LPO and neutrophilic phagocytic activity .
	manualset3
171549	1	413264	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There were , in all patients , mean increases in peripheral vascular resistance from period 1 to period 2 of 239 ( 95 % confidence interval 135 , 343 ) dynes.sec.cm-5 , from period 2 to period 3 of 85 ( -64 , 234 ) dynes.sec.cm-5 , and from period 1 to period 3 of 324 ( 95 % confidence interval 175 , 473 ) dynes.sec.cm-5 .
	manualset3
171550	2	413264	7	NULL	NULL	0	NULL	mean increases	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There were , in all patients , mean increases in peripheral vascular resistance from period 1 to period 2 of 239 ( 95 % confidence interval 135 , 343 ) dynes.sec.cm-5 , from period 2 to period 3 of 85 ( -64 , 234 ) dynes.sec.cm-5 , and from period 1 to period 3 of 324 ( 95 % confidence interval 175 , 473 ) dynes.sec.cm-5 .
	manualset3
171551	3	413264	7	NULL	NULL	0	NULL	peripheral vascular resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There were , in all patients , mean increases in peripheral vascular resistance from period 1 to period 2 of 239 ( 95 % confidence interval 135 , 343 ) dynes.sec.cm-5 , from period 2 to period 3 of 85 ( -64 , 234 ) dynes.sec.cm-5 , and from period 1 to period 3 of 324 ( 95 % confidence interval 175 , 473 ) dynes.sec.cm-5 .
	manualset3
171552	4	413264	7	NULL	NULL	0	NULL	period 1 to period 2	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	There were , in all patients , mean increases in peripheral vascular resistance from period 1 to period 2 of 239 ( 95 % confidence interval 135 , 343 ) dynes.sec.cm-5 , from period 2 to period 3 of 85 ( -64 , 234 ) dynes.sec.cm-5 , and from period 1 to period 3 of 324 ( 95 % confidence interval 175 , 473 ) dynes.sec.cm-5 .
	manualset3
171553	5	413264	7	NULL	NULL	NULL	NULL	239 dynes.sec.cm-5	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There were , in all patients , mean increases in peripheral vascular resistance from period 1 to period 2 of 239 ( 95 % confidence interval 135 , 343 ) dynes.sec.cm-5 , from period 2 to period 3 of 85 ( -64 , 234 ) dynes.sec.cm-5 , and from period 1 to period 3 of 324 ( 95 % confidence interval 175 , 473 ) dynes.sec.cm-5 .
	manualset3
171554	6	413264	7	NULL	NULL	0	NULL	95 % confidence interval 135 , 343	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There were , in all patients , mean increases in peripheral vascular resistance from period 1 to period 2 of 239 ( 95 % confidence interval 135 , 343 ) dynes.sec.cm-5 , from period 2 to period 3 of 85 ( -64 , 234 ) dynes.sec.cm-5 , and from period 1 to period 3 of 324 ( 95 % confidence interval 175 , 473 ) dynes.sec.cm-5 .
	manualset3
171555	7	413264	7	NULL	NULL	0	NULL	period 2 to period 3 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	There were , in all patients , mean increases in peripheral vascular resistance from period 1 to period 2 of 239 ( 95 % confidence interval 135 , 343 ) dynes.sec.cm-5 , from period 2 to period 3 of 85 ( -64 , 234 ) dynes.sec.cm-5 , and from period 1 to period 3 of 324 ( 95 % confidence interval 175 , 473 ) dynes.sec.cm-5 .
	manualset3
171556	8	413264	7	NULL	NULL	0	NULL	85 dynes.sec.cm-5	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There were , in all patients , mean increases in peripheral vascular resistance from period 1 to period 2 of 239 ( 95 % confidence interval 135 , 343 ) dynes.sec.cm-5 , from period 2 to period 3 of 85 ( -64 , 234 ) dynes.sec.cm-5 , and from period 1 to period 3 of 324 ( 95 % confidence interval 175 , 473 ) dynes.sec.cm-5 .
	manualset3
171557	9	413264	7	NULL	NULL	0	NULL	-64 , 234	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There were , in all patients , mean increases in peripheral vascular resistance from period 1 to period 2 of 239 ( 95 % confidence interval 135 , 343 ) dynes.sec.cm-5 , from period 2 to period 3 of 85 ( -64 , 234 ) dynes.sec.cm-5 , and from period 1 to period 3 of 324 ( 95 % confidence interval 175 , 473 ) dynes.sec.cm-5 .
	manualset3
171558	10	413264	7	NULL	NULL	0	NULL	period 1 to period 3	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	There were , in all patients , mean increases in peripheral vascular resistance from period 1 to period 2 of 239 ( 95 % confidence interval 135 , 343 ) dynes.sec.cm-5 , from period 2 to period 3 of 85 ( -64 , 234 ) dynes.sec.cm-5 , and from period 1 to period 3 of 324 ( 95 % confidence interval 175 , 473 ) dynes.sec.cm-5 .
	manualset3
171559	11	413264	7	NULL	NULL	0	NULL	324 dynes.sec.cm-5	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There were , in all patients , mean increases in peripheral vascular resistance from period 1 to period 2 of 239 ( 95 % confidence interval 135 , 343 ) dynes.sec.cm-5 , from period 2 to period 3 of 85 ( -64 , 234 ) dynes.sec.cm-5 , and from period 1 to period 3 of 324 ( 95 % confidence interval 175 , 473 ) dynes.sec.cm-5 .
	manualset3
171560	12	413264	7	NULL	NULL	0	NULL	95 % confidence interval 175 , 473	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There were , in all patients , mean increases in peripheral vascular resistance from period 1 to period 2 of 239 ( 95 % confidence interval 135 , 343 ) dynes.sec.cm-5 , from period 2 to period 3 of 85 ( -64 , 234 ) dynes.sec.cm-5 , and from period 1 to period 3 of 324 ( 95 % confidence interval 175 , 473 ) dynes.sec.cm-5 .
	manualset3
171561	1	413265	7	NULL	NULL	0	NULL	11 positive tests	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 11 positive tests , including confirmatory positives on 2 persons diagnosed by colonoscopy , and to date surgery has been successfully undertaken on 3 previously undiagnosed adults .
	manualset3
171562	2	413265	7	NULL	NULL	0	NULL	confirmatory positives	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 11 positive tests , including confirmatory positives on 2 persons diagnosed by colonoscopy , and to date surgery has been successfully undertaken on 3 previously undiagnosed adults .
	manualset3
171563	3	413265	7	NULL	NULL	0	NULL	2 persons	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 11 positive tests , including confirmatory positives on 2 persons diagnosed by colonoscopy , and to date surgery has been successfully undertaken on 3 previously undiagnosed adults .
	manualset3
171564	4	413265	7	NULL	NULL	0	NULL	colonoscopy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 11 positive tests , including confirmatory positives on 2 persons diagnosed by colonoscopy , and to date surgery has been successfully undertaken on 3 previously undiagnosed adults .
	manualset3
171565	5	413265	7	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 11 positive tests , including confirmatory positives on 2 persons diagnosed by colonoscopy , and to date surgery has been successfully undertaken on 3 previously undiagnosed adults .
	manualset3
171566	6	413265	7	NULL	NULL	0	NULL	 3 previously undiagnosed adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 11 positive tests , including confirmatory positives on 2 persons diagnosed by colonoscopy , and to date surgery has been successfully undertaken on 3 previously undiagnosed adults .
	manualset3
171567	1	413266	7	NULL	NULL	0	NULL	155 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 155 cases ( 16.0 % ) of 3 vessel disease , 154 cases ( 15.9 % ) of 2 vessel disease , 215 cases ( 22.2 % ) of 1 vessel disease , and 444 cases ( 45.9 % ) of no significant coronary sclerosis .
	manualset3
171568	2	413266	7	NULL	NULL	0	NULL	16.0 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 155 cases ( 16.0 % ) of 3 vessel disease , 154 cases ( 15.9 % ) of 2 vessel disease , 215 cases ( 22.2 % ) of 1 vessel disease , and 444 cases ( 45.9 % ) of no significant coronary sclerosis .
	manualset3
171569	3	413266	7	NULL	NULL	0	NULL	3 vessel disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 155 cases ( 16.0 % ) of 3 vessel disease , 154 cases ( 15.9 % ) of 2 vessel disease , 215 cases ( 22.2 % ) of 1 vessel disease , and 444 cases ( 45.9 % ) of no significant coronary sclerosis .
	manualset3
171570	4	413266	7	NULL	NULL	0	NULL	154 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 155 cases ( 16.0 % ) of 3 vessel disease , 154 cases ( 15.9 % ) of 2 vessel disease , 215 cases ( 22.2 % ) of 1 vessel disease , and 444 cases ( 45.9 % ) of no significant coronary sclerosis .
	manualset3
171571	5	413266	7	NULL	NULL	0	NULL	15.9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 155 cases ( 16.0 % ) of 3 vessel disease , 154 cases ( 15.9 % ) of 2 vessel disease , 215 cases ( 22.2 % ) of 1 vessel disease , and 444 cases ( 45.9 % ) of no significant coronary sclerosis .
	manualset3
171572	6	413266	7	NULL	NULL	0	NULL	2 vessel disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 155 cases ( 16.0 % ) of 3 vessel disease , 154 cases ( 15.9 % ) of 2 vessel disease , 215 cases ( 22.2 % ) of 1 vessel disease , and 444 cases ( 45.9 % ) of no significant coronary sclerosis .
	manualset3
171573	7	413266	7	NULL	NULL	0	NULL	215 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 155 cases ( 16.0 % ) of 3 vessel disease , 154 cases ( 15.9 % ) of 2 vessel disease , 215 cases ( 22.2 % ) of 1 vessel disease , and 444 cases ( 45.9 % ) of no significant coronary sclerosis .
	manualset3
171574	8	413266	7	NULL	NULL	0	NULL	22.2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 155 cases ( 16.0 % ) of 3 vessel disease , 154 cases ( 15.9 % ) of 2 vessel disease , 215 cases ( 22.2 % ) of 1 vessel disease , and 444 cases ( 45.9 % ) of no significant coronary sclerosis .
	manualset3
171575	9	413266	7	NULL	NULL	0	NULL	1 vessel disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 155 cases ( 16.0 % ) of 3 vessel disease , 154 cases ( 15.9 % ) of 2 vessel disease , 215 cases ( 22.2 % ) of 1 vessel disease , and 444 cases ( 45.9 % ) of no significant coronary sclerosis .
	manualset3
171576	10	413266	7	NULL	NULL	0	NULL	444 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 155 cases ( 16.0 % ) of 3 vessel disease , 154 cases ( 15.9 % ) of 2 vessel disease , 215 cases ( 22.2 % ) of 1 vessel disease , and 444 cases ( 45.9 % ) of no significant coronary sclerosis .
	manualset3
171577	11	413266	7	NULL	NULL	0	NULL	45.9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 155 cases ( 16.0 % ) of 3 vessel disease , 154 cases ( 15.9 % ) of 2 vessel disease , 215 cases ( 22.2 % ) of 1 vessel disease , and 444 cases ( 45.9 % ) of no significant coronary sclerosis .
	manualset3
171578	12	413266	7	NULL	NULL	0	NULL	no significant coronary sclerosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 155 cases ( 16.0 % ) of 3 vessel disease , 154 cases ( 15.9 % ) of 2 vessel disease , 215 cases ( 22.2 % ) of 1 vessel disease , and 444 cases ( 45.9 % ) of no significant coronary sclerosis .
	manualset3
171579	1	413267	7	NULL	NULL	0	NULL	Activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity in the partial reactions correlated with intrinsic fluorescence enhancement of tryptophan residues in either the 12 S or 5 S subunit .
	manualset3
171580	2	413267	7	NULL	NULL	0	NULL	partial reactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity in the partial reactions correlated with intrinsic fluorescence enhancement of tryptophan residues in either the 12 S or 5 S subunit .
	manualset3
171581	3	413267	7	NULL	NULL	0	NULL	intrinsic fluorescence enhancement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity in the partial reactions correlated with intrinsic fluorescence enhancement of tryptophan residues in either the 12 S or 5 S subunit .
	manualset3
171582	4	413267	7	NULL	NULL	0	NULL	tryptophan residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity in the partial reactions correlated with intrinsic fluorescence enhancement of tryptophan residues in either the 12 S or 5 S subunit .
	manualset3
171583	5	413267	7	NULL	NULL	0	NULL	12 S subunit	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity in the partial reactions correlated with intrinsic fluorescence enhancement of tryptophan residues in either the 12 S or 5 S subunit .
	manualset3
171584	6	413267	7	NULL	NULL	0	NULL	5 S subunit	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity in the partial reactions correlated with intrinsic fluorescence enhancement of tryptophan residues in either the 12 S or 5 S subunit .
	manualset3
171585	1	413268	7	NULL	NULL	0	NULL	3 classes	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 3 classes with relative correspondence between height and weight : 1 .
	manualset3
171586	2	413268	7	NULL	NULL	0	NULL	relative correspondence	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 3 classes with relative correspondence between height and weight : 1 .
	manualset3
171587	3	413268	7	NULL	NULL	0	NULL	 height	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 3 classes with relative correspondence between height and weight : 1 .
	manualset3
171588	4	413268	7	NULL	NULL	0	NULL	weight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 3 classes with relative correspondence between height and weight : 1 .
	manualset3
171589	5	413268	7	NULL	NULL	0	NULL	 1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 3 classes with relative correspondence between height and weight : 1 .
	manualset3
171590	1	413269	7	NULL	NULL	0	NULL	3 epidemic outbreaks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 3 epidemic outbreaks : Coxsackievirus A9 ( 1990-1991 ) , Echovirus 30 ( 1994 ) , and Coxsackievirus B5 ( 1995 ) .
	manualset3
171591	2	413269	7	NULL	NULL	0	NULL	Coxsackievirus A9	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 3 epidemic outbreaks : Coxsackievirus A9 ( 1990-1991 ) , Echovirus 30 ( 1994 ) , and Coxsackievirus B5 ( 1995 ) .
	manualset3
171592	3	413269	7	NULL	NULL	0	NULL	1990-1991	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 3 epidemic outbreaks : Coxsackievirus A9 ( 1990-1991 ) , Echovirus 30 ( 1994 ) , and Coxsackievirus B5 ( 1995 ) .
	manualset3
171593	4	413269	7	NULL	NULL	0	NULL	Echovirus 30	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 3 epidemic outbreaks : Coxsackievirus A9 ( 1990-1991 ) , Echovirus 30 ( 1994 ) , and Coxsackievirus B5 ( 1995 ) .
	manualset3
171594	5	413269	7	NULL	NULL	0	NULL	1994	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 3 epidemic outbreaks : Coxsackievirus A9 ( 1990-1991 ) , Echovirus 30 ( 1994 ) , and Coxsackievirus B5 ( 1995 ) .
	manualset3
171595	6	413269	7	NULL	NULL	0	NULL	Coxsackievirus B5	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 3 epidemic outbreaks : Coxsackievirus A9 ( 1990-1991 ) , Echovirus 30 ( 1994 ) , and Coxsackievirus B5 ( 1995 ) .
	manualset3
171596	7	413269	7	NULL	NULL	0	NULL	1995	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 3 epidemic outbreaks : Coxsackievirus A9 ( 1990-1991 ) , Echovirus 30 ( 1994 ) , and Coxsackievirus B5 ( 1995 ) .
	manualset3
171597	1	413270	7	NULL	NULL	0	NULL	54 recognized species 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 54 recognized species of this genus , associated with marine or saline sites .
	manualset3
171598	2	413270	7	NULL	NULL	0	NULL	genus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 54 recognized species of this genus , associated with marine or saline sites .
	manualset3
171599	3	413270	7	NULL	NULL	0	NULL	marine or saline sites	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	There were 54 recognized species of this genus , associated with marine or saline sites .
	manualset3
171600	1	413271	7	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There were also considerable differences between the distributions of substitutions within the SUP4-o gene .
	manualset3
171601	2	413271	7	NULL	NULL	0	NULL	distributions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There were also considerable differences between the distributions of substitutions within the SUP4-o gene .
	manualset3
171602	3	413271	7	NULL	NULL	0	NULL	substitutions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There were also considerable differences between the distributions of substitutions within the SUP4-o gene .
	manualset3
171603	4	413271	7	NULL	NULL	0	NULL	SUP4-o gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	There were also considerable differences between the distributions of substitutions within the SUP4-o gene .
	manualset3
171604	1	413272	7	NULL	NULL	0	NULL	minor amounts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There were also minor amounts of ( 1a , 2a , 3a ) collagen , and , in the two denser fractions , of type I collagen .
	manualset3
171605	2	413272	7	NULL	NULL	0	NULL	( 1a , 2a , 3a ) collagen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	There were also minor amounts of ( 1a , 2a , 3a ) collagen , and , in the two denser fractions , of type I collagen .
	manualset3
171606	3	413272	7	NULL	NULL	0	NULL	two denser fractions	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There were also minor amounts of ( 1a , 2a , 3a ) collagen , and , in the two denser fractions , of type I collagen .
	manualset3
171607	4	413272	7	NULL	NULL	0	NULL	type I collagen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	There were also minor amounts of ( 1a , 2a , 3a ) collagen , and , in the two denser fractions , of type I collagen .
	manualset3
171608	1	413273	7	NULL	NULL	0	NULL	associations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There were associations between prepubertal GH parameters , glucose and non-esterified fatty acid ( NEFA ) concentrations and the body condition score at which the animals attained puberty .
	manualset3
171609	2	413273	7	NULL	NULL	0	NULL	prepubertal GH parameters	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There were associations between prepubertal GH parameters , glucose and non-esterified fatty acid ( NEFA ) concentrations and the body condition score at which the animals attained puberty .
	manualset3
171610	3	413273	7	NULL	NULL	0	NULL	glucose	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	There were associations between prepubertal GH parameters , glucose and non-esterified fatty acid ( NEFA ) concentrations and the body condition score at which the animals attained puberty .
	manualset3
171611	4	413273	7	NULL	NULL	0	NULL	non-esterified fatty acid ( NEFA ) concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There were associations between prepubertal GH parameters , glucose and non-esterified fatty acid ( NEFA ) concentrations and the body condition score at which the animals attained puberty .
	manualset3
171612	5	413273	7	NULL	NULL	0	NULL	body condition score	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were associations between prepubertal GH parameters , glucose and non-esterified fatty acid ( NEFA ) concentrations and the body condition score at which the animals attained puberty .
	manualset3
171613	6	413273	7	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	There were associations between prepubertal GH parameters , glucose and non-esterified fatty acid ( NEFA ) concentrations and the body condition score at which the animals attained puberty .
	manualset3
171614	7	413273	7	NULL	NULL	0	NULL	puberty	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There were associations between prepubertal GH parameters , glucose and non-esterified fatty acid ( NEFA ) concentrations and the body condition score at which the animals attained puberty .
	manualset3
171615	1	413274	7	NULL	NULL	0	NULL	clinical manifestations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were following clinical manifestations : common symptoms of the infection ; acute uveitis ( rapid focal iridic destruction , pupillary deformities , formation of membranes in the anterior chamber of the eye ) ; and in 15-30 % of cases severe complications , cataract , glaucoma , vision impairments .
	manualset3
171616	2	413274	7	NULL	NULL	0	NULL	common symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were following clinical manifestations : common symptoms of the infection ; acute uveitis ( rapid focal iridic destruction , pupillary deformities , formation of membranes in the anterior chamber of the eye ) ; and in 15-30 % of cases severe complications , cataract , glaucoma , vision impairments .
	manualset3
171617	3	413274	7	NULL	NULL	0	NULL	infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were following clinical manifestations : common symptoms of the infection ; acute uveitis ( rapid focal iridic destruction , pupillary deformities , formation of membranes in the anterior chamber of the eye ) ; and in 15-30 % of cases severe complications , cataract , glaucoma , vision impairments .
	manualset3
171618	4	413274	7	NULL	NULL	0	NULL	 acute uveitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were following clinical manifestations : common symptoms of the infection ; acute uveitis ( rapid focal iridic destruction , pupillary deformities , formation of membranes in the anterior chamber of the eye ) ; and in 15-30 % of cases severe complications , cataract , glaucoma , vision impairments .
	manualset3
171619	5	413274	7	NULL	NULL	0	NULL	rapid focal iridic destruction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were following clinical manifestations : common symptoms of the infection ; acute uveitis ( rapid focal iridic destruction , pupillary deformities , formation of membranes in the anterior chamber of the eye ) ; and in 15-30 % of cases severe complications , cataract , glaucoma , vision impairments .
	manualset3
171620	6	413274	7	NULL	NULL	0	NULL	pupillary deformities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were following clinical manifestations : common symptoms of the infection ; acute uveitis ( rapid focal iridic destruction , pupillary deformities , formation of membranes in the anterior chamber of the eye ) ; and in 15-30 % of cases severe complications , cataract , glaucoma , vision impairments .
	manualset3
171621	7	413274	7	NULL	NULL	0	NULL	formation of membranes in the anterior chamber of the eye	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were following clinical manifestations : common symptoms of the infection ; acute uveitis ( rapid focal iridic destruction , pupillary deformities , formation of membranes in the anterior chamber of the eye ) ; and in 15-30 % of cases severe complications , cataract , glaucoma , vision impairments .
	manualset3
171622	8	413274	7	NULL	NULL	0	NULL	15-30 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There were following clinical manifestations : common symptoms of the infection ; acute uveitis ( rapid focal iridic destruction , pupillary deformities , formation of membranes in the anterior chamber of the eye ) ; and in 15-30 % of cases severe complications , cataract , glaucoma , vision impairments .
	manualset3
171623	9	413274	7	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There were following clinical manifestations : common symptoms of the infection ; acute uveitis ( rapid focal iridic destruction , pupillary deformities , formation of membranes in the anterior chamber of the eye ) ; and in 15-30 % of cases severe complications , cataract , glaucoma , vision impairments .
	manualset3
171624	10	413274	7	NULL	NULL	0	NULL	complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were following clinical manifestations : common symptoms of the infection ; acute uveitis ( rapid focal iridic destruction , pupillary deformities , formation of membranes in the anterior chamber of the eye ) ; and in 15-30 % of cases severe complications , cataract , glaucoma , vision impairments .
	manualset3
171625	11	413274	7	NULL	NULL	0	NULL	cataract	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were following clinical manifestations : common symptoms of the infection ; acute uveitis ( rapid focal iridic destruction , pupillary deformities , formation of membranes in the anterior chamber of the eye ) ; and in 15-30 % of cases severe complications , cataract , glaucoma , vision impairments .
	manualset3
171626	12	413274	7	NULL	NULL	0	NULL	glaucoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were following clinical manifestations : common symptoms of the infection ; acute uveitis ( rapid focal iridic destruction , pupillary deformities , formation of membranes in the anterior chamber of the eye ) ; and in 15-30 % of cases severe complications , cataract , glaucoma , vision impairments .
	manualset3
171627	13	413274	7	NULL	NULL	0	NULL	vision impairments	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were following clinical manifestations : common symptoms of the infection ; acute uveitis ( rapid focal iridic destruction , pupillary deformities , formation of membranes in the anterior chamber of the eye ) ; and in 15-30 % of cases severe complications , cataract , glaucoma , vision impairments .
	manualset3
171628	1	413275	7	NULL	NULL	0	NULL	modest	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were modest but significant positive associations between attachment anxiety and both severity and distress in relation to voice hearing , but no associations between attachment avoidance and these dimensions .
	manualset3
171629	2	413275	7	NULL	NULL	0	NULL	positive associations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There were modest but significant positive associations between attachment anxiety and both severity and distress in relation to voice hearing , but no associations between attachment avoidance and these dimensions .
	manualset3
171630	3	413275	7	NULL	NULL	0	NULL	 attachment anxiety	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were modest but significant positive associations between attachment anxiety and both severity and distress in relation to voice hearing , but no associations between attachment avoidance and these dimensions .
	manualset3
171631	4	413275	7	NULL	NULL	0	NULL	severity and distress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were modest but significant positive associations between attachment anxiety and both severity and distress in relation to voice hearing , but no associations between attachment avoidance and these dimensions .
	manualset3
171632	5	413275	7	NULL	NULL	0	NULL	 relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There were modest but significant positive associations between attachment anxiety and both severity and distress in relation to voice hearing , but no associations between attachment avoidance and these dimensions .
	manualset3
171633	6	413275	7	NULL	NULL	0	NULL	voice hearing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were modest but significant positive associations between attachment anxiety and both severity and distress in relation to voice hearing , but no associations between attachment avoidance and these dimensions .
	manualset3
171634	7	413275	7	NULL	NULL	0	NULL	no associations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There were modest but significant positive associations between attachment anxiety and both severity and distress in relation to voice hearing , but no associations between attachment avoidance and these dimensions .
	manualset3
171635	8	413275	7	NULL	NULL	0	NULL	attachment avoidance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were modest but significant positive associations between attachment anxiety and both severity and distress in relation to voice hearing , but no associations between attachment avoidance and these dimensions .
	manualset3
171636	9	413275	7	NULL	NULL	0	NULL	dimensions	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There were modest but significant positive associations between attachment anxiety and both severity and distress in relation to voice hearing , but no associations between attachment avoidance and these dimensions .
	manualset3
171637	1	413276	7	NULL	NULL	0	NULL	no correlations 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no correlations between CB1R binding and any predefined migraine characteristics .
	manualset3
171638	2	413276	7	NULL	NULL	0	NULL	CB1R binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no correlations between CB1R binding and any predefined migraine characteristics .
	manualset3
171639	3	413276	7	NULL	NULL	0	NULL	migraine characteristics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no correlations between CB1R binding and any predefined migraine characteristics .
	manualset3
171640	1	413277	7	NULL	NULL	0	NULL	no deaths	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no deaths , and patients treated as an emergency with plasma expanders or with adrenaline and corticosteroids generally recovered promptly and uneventfully .
	manualset3
171641	2	413277	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no deaths , and patients treated as an emergency with plasma expanders or with adrenaline and corticosteroids generally recovered promptly and uneventfully .
	manualset3
171642	3	413277	7	NULL	NULL	0	NULL	 emergency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no deaths , and patients treated as an emergency with plasma expanders or with adrenaline and corticosteroids generally recovered promptly and uneventfully .
	manualset3
171643	4	413277	7	NULL	NULL	0	NULL	plasma expanders	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no deaths , and patients treated as an emergency with plasma expanders or with adrenaline and corticosteroids generally recovered promptly and uneventfully .
	manualset3
171644	5	413277	7	NULL	NULL	0	NULL	adrenaline	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no deaths , and patients treated as an emergency with plasma expanders or with adrenaline and corticosteroids generally recovered promptly and uneventfully .
	manualset3
171645	6	413277	7	NULL	NULL	0	NULL	corticosteroids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no deaths , and patients treated as an emergency with plasma expanders or with adrenaline and corticosteroids generally recovered promptly and uneventfully .
	manualset3
171646	1	413278	7	NULL	NULL	0	NULL	Activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity of aspartate transcarbamylase in uninfected and type 5 adenovirus-infected HeLa cells .
	manualset3
171647	2	413278	7	NULL	NULL	0	NULL	aspartate transcarbamylase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity of aspartate transcarbamylase in uninfected and type 5 adenovirus-infected HeLa cells .
	manualset3
171648	3	413278	7	NULL	NULL	0	NULL	type 5 adenovirus-infected HeLa cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity of aspartate transcarbamylase in uninfected and type 5 adenovirus-infected HeLa cells .
	manualset3
171649	1	413279	7	NULL	NULL	0	NULL	no differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no differences in preterm birth between neighborhood deprivation tertiles among immigrants with less than 15years of residence .
	manualset3
171650	2	413279	7	NULL	NULL	0	NULL	preterm birth 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no differences in preterm birth between neighborhood deprivation tertiles among immigrants with less than 15years of residence .
	manualset3
171651	3	413279	7	NULL	NULL	0	NULL	 neighborhood deprivation	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no differences in preterm birth between neighborhood deprivation tertiles among immigrants with less than 15years of residence .
	manualset3
171652	4	413279	7	NULL	NULL	0	NULL	immigrants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no differences in preterm birth between neighborhood deprivation tertiles among immigrants with less than 15years of residence .
	manualset3
171653	5	413279	7	NULL	NULL	0	NULL	15years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no differences in preterm birth between neighborhood deprivation tertiles among immigrants with less than 15years of residence .
	manualset3
171654	6	413279	7	NULL	NULL	0	NULL	residence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no differences in preterm birth between neighborhood deprivation tertiles among immigrants with less than 15years of residence .
	manualset3
171655	1	413280	7	NULL	NULL	0	NULL	 no differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no differences in the timing of brood desertion between experimental and control females in an experiment in which we lengthened or shortened the duration of incubation by one week .
	manualset3
171656	2	413280	7	NULL	NULL	0	NULL	timing	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no differences in the timing of brood desertion between experimental and control females in an experiment in which we lengthened or shortened the duration of incubation by one week .
	manualset3
171657	3	413280	7	NULL	NULL	0	NULL	brood desertion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no differences in the timing of brood desertion between experimental and control females in an experiment in which we lengthened or shortened the duration of incubation by one week .
	manualset3
171658	4	413280	7	NULL	NULL	0	NULL	 experimental females	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no differences in the timing of brood desertion between experimental and control females in an experiment in which we lengthened or shortened the duration of incubation by one week .
	manualset3
171659	5	413280	7	NULL	NULL	0	NULL	control females	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no differences in the timing of brood desertion between experimental and control females in an experiment in which we lengthened or shortened the duration of incubation by one week .
	manualset3
171660	6	413280	7	NULL	NULL	0	NULL	experiment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no differences in the timing of brood desertion between experimental and control females in an experiment in which we lengthened or shortened the duration of incubation by one week .
	manualset3
171661	7	413280	7	NULL	NULL	0	NULL	duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no differences in the timing of brood desertion between experimental and control females in an experiment in which we lengthened or shortened the duration of incubation by one week .
	manualset3
171662	8	413280	7	NULL	NULL	0	NULL	incubation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no differences in the timing of brood desertion between experimental and control females in an experiment in which we lengthened or shortened the duration of incubation by one week .
	manualset3
171663	9	413280	7	NULL	NULL	0	NULL	one week	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no differences in the timing of brood desertion between experimental and control females in an experiment in which we lengthened or shortened the duration of incubation by one week .
	manualset3
171664	1	413281	7	NULL	NULL	0	NULL	no significant associations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant associations between receipt of rituximab and the factors analyzed .
	manualset3
171665	2	413281	7	NULL	NULL	0	NULL	receipt 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant associations between receipt of rituximab and the factors analyzed .
	manualset3
171666	3	413281	7	NULL	NULL	0	NULL	rituximab	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant associations between receipt of rituximab and the factors analyzed .
	manualset3
171667	4	413281	7	NULL	NULL	0	NULL	factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant associations between receipt of rituximab and the factors analyzed .
	manualset3
171668	1	413282	7	NULL	NULL	NULL	NULL	no significant changes	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There were no significant changes in I-labelled BSA recorded on the charcoal before and after in vivo procedures and no signifcant alterations in hematocrit , serum sodium , potassium , calcium , magnesium or creatinine levels before and after the procedures .
	manualset3
171669	2	413282	7	NULL	NULL	0	NULL	I-labelled BSA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant changes in I-labelled BSA recorded on the charcoal before and after in vivo procedures and no signifcant alterations in hematocrit , serum sodium , potassium , calcium , magnesium or creatinine levels before and after the procedures .
	manualset3
171670	3	413282	7	NULL	NULL	0	NULL	charcoal	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant changes in I-labelled BSA recorded on the charcoal before and after in vivo procedures and no signifcant alterations in hematocrit , serum sodium , potassium , calcium , magnesium or creatinine levels before and after the procedures .
	manualset3
171672	4	413282	7	NULL	NULL	0	NULL	in vivo procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant changes in I-labelled BSA recorded on the charcoal before and after in vivo procedures and no signifcant alterations in hematocrit , serum sodium , potassium , calcium , magnesium or creatinine levels before and after the procedures .
	manualset3
171673	5	413282	7	NULL	NULL	0	NULL	no signifcant alterations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant changes in I-labelled BSA recorded on the charcoal before and after in vivo procedures and no signifcant alterations in hematocrit , serum sodium , potassium , calcium , magnesium or creatinine levels before and after the procedures .
	manualset3
171674	6	413282	7	NULL	NULL	0	NULL	 hematocrit	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant changes in I-labelled BSA recorded on the charcoal before and after in vivo procedures and no signifcant alterations in hematocrit , serum sodium , potassium , calcium , magnesium or creatinine levels before and after the procedures .
	manualset3
171675	7	413282	7	NULL	NULL	NULL	NULL	serum sodium 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There were no significant changes in I-labelled BSA recorded on the charcoal before and after in vivo procedures and no signifcant alterations in hematocrit , serum sodium , potassium , calcium , magnesium or creatinine levels before and after the procedures .
	manualset3
171676	8	413282	7	NULL	NULL	0	NULL	potassium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant changes in I-labelled BSA recorded on the charcoal before and after in vivo procedures and no signifcant alterations in hematocrit , serum sodium , potassium , calcium , magnesium or creatinine levels before and after the procedures .
	manualset3
171677	9	413282	7	NULL	NULL	0	NULL	calcium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant changes in I-labelled BSA recorded on the charcoal before and after in vivo procedures and no signifcant alterations in hematocrit , serum sodium , potassium , calcium , magnesium or creatinine levels before and after the procedures .
	manualset3
171678	10	413282	7	NULL	NULL	0	NULL	magnesium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant changes in I-labelled BSA recorded on the charcoal before and after in vivo procedures and no signifcant alterations in hematocrit , serum sodium , potassium , calcium , magnesium or creatinine levels before and after the procedures .
	manualset3
171679	11	413282	7	NULL	NULL	0	NULL	creatinine levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant changes in I-labelled BSA recorded on the charcoal before and after in vivo procedures and no signifcant alterations in hematocrit , serum sodium , potassium , calcium , magnesium or creatinine levels before and after the procedures .
	manualset3
171680	12	413282	7	NULL	NULL	0	NULL	procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant changes in I-labelled BSA recorded on the charcoal before and after in vivo procedures and no signifcant alterations in hematocrit , serum sodium , potassium , calcium , magnesium or creatinine levels before and after the procedures .
	manualset3
171681	1	413283	7	NULL	NULL	0	NULL	 no significant changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant changes in plasma levels of histamine or catecholamines .
	manualset3
171682	2	413283	7	NULL	NULL	0	NULL	plasma levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant changes in plasma levels of histamine or catecholamines .
	manualset3
171683	3	413283	7	NULL	NULL	0	NULL	histamine	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant changes in plasma levels of histamine or catecholamines .
	manualset3
171684	4	413283	7	NULL	NULL	0	NULL	catecholamines	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant changes in plasma levels of histamine or catecholamines .
	manualset3
171685	1	413284	7	NULL	NULL	0	NULL	Activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity of enzymes involved in the bactericidal properties of neutrophils and their capacity to reduce nitroblue tetrazolium were studied in 60 patients with acute myeloblastic leukemia ( AML ) .
	manualset3
171686	2	413284	7	NULL	NULL	0	NULL	 enzymes	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity of enzymes involved in the bactericidal properties of neutrophils and their capacity to reduce nitroblue tetrazolium were studied in 60 patients with acute myeloblastic leukemia ( AML ) .
	manualset3
171687	3	413284	7	NULL	NULL	0	NULL	bactericidal properties	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity of enzymes involved in the bactericidal properties of neutrophils and their capacity to reduce nitroblue tetrazolium were studied in 60 patients with acute myeloblastic leukemia ( AML ) .
	manualset3
171688	4	413284	7	NULL	NULL	0	NULL	neutrophils	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity of enzymes involved in the bactericidal properties of neutrophils and their capacity to reduce nitroblue tetrazolium were studied in 60 patients with acute myeloblastic leukemia ( AML ) .
	manualset3
171689	5	413284	7	NULL	NULL	0	NULL	capacity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity of enzymes involved in the bactericidal properties of neutrophils and their capacity to reduce nitroblue tetrazolium were studied in 60 patients with acute myeloblastic leukemia ( AML ) .
	manualset3
171690	6	413284	7	NULL	NULL	0	NULL	nitroblue tetrazolium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity of enzymes involved in the bactericidal properties of neutrophils and their capacity to reduce nitroblue tetrazolium were studied in 60 patients with acute myeloblastic leukemia ( AML ) .
	manualset3
171691	7	413284	7	NULL	NULL	0	NULL	60 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity of enzymes involved in the bactericidal properties of neutrophils and their capacity to reduce nitroblue tetrazolium were studied in 60 patients with acute myeloblastic leukemia ( AML ) .
	manualset3
171692	8	413284	7	NULL	NULL	0	NULL	acute myeloblastic leukemia ( AML ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity of enzymes involved in the bactericidal properties of neutrophils and their capacity to reduce nitroblue tetrazolium were studied in 60 patients with acute myeloblastic leukemia ( AML ) .
	manualset3
171693	1	413285	7	NULL	NULL	0	NULL	no significant correlations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant correlations between the immunohistochemical stainings for neuron-specific enolase and keratin and the clinical characteristics in these cases .
	manualset3
171694	2	413285	7	NULL	NULL	0	NULL	immunohistochemical stainings 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant correlations between the immunohistochemical stainings for neuron-specific enolase and keratin and the clinical characteristics in these cases .
	manualset3
171695	3	413285	7	NULL	NULL	0	NULL	neuron-specific enolase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant correlations between the immunohistochemical stainings for neuron-specific enolase and keratin and the clinical characteristics in these cases .
	manualset3
171696	4	413285	7	NULL	NULL	0	NULL	 keratin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant correlations between the immunohistochemical stainings for neuron-specific enolase and keratin and the clinical characteristics in these cases .
	manualset3
171697	5	413285	7	NULL	NULL	0	NULL	 clinical characteristics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant correlations between the immunohistochemical stainings for neuron-specific enolase and keratin and the clinical characteristics in these cases .
	manualset3
171698	1	413286	7	NULL	NULL	0	NULL	no significant differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences between VE and PL in muscle soreness , performance measures , or plasma MDA .
	manualset3
171699	2	413286	7	NULL	NULL	0	NULL	 VE	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences between VE and PL in muscle soreness , performance measures , or plasma MDA .
	manualset3
171700	3	413286	7	NULL	NULL	0	NULL	PL	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences between VE and PL in muscle soreness , performance measures , or plasma MDA .
	manualset3
171701	4	413286	7	NULL	NULL	0	NULL	muscle soreness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences between VE and PL in muscle soreness , performance measures , or plasma MDA .
	manualset3
171702	5	413286	7	NULL	NULL	0	NULL	measures	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences between VE and PL in muscle soreness , performance measures , or plasma MDA .
	manualset3
171703	6	413286	7	NULL	NULL	0	NULL	plasma MDA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences between VE and PL in muscle soreness , performance measures , or plasma MDA .
	manualset3
171704	1	413287	7	NULL	NULL	0	NULL	no significant differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences between the MIDCAB group and the off-pump group in age , being 57 + / - 11 vs 66 + / - 8 years old , the operative time , being 321 + / - 149 vs 441 + / - 205 min , the number of grafts , being 1.0 vs 1.4 / patient , peak creatine kinase ( CK ) values , being 662 + / - 436 vs 609 + / - 56 IU/l , the peak CK-muscle-brain values , being 12 + / - 9 vs 16 + / - 5 IU/l , and the postoperative blood loss , being 369 + / - 198 vs 541 + / - 204 ml .
	manualset3
171705	2	413287	7	NULL	NULL	0	NULL	MIDCAB group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences between the MIDCAB group and the off-pump group in age , being 57 + / - 11 vs 66 + / - 8 years old , the operative time , being 321 + / - 149 vs 441 + / - 205 min , the number of grafts , being 1.0 vs 1.4 / patient , peak creatine kinase ( CK ) values , being 662 + / - 436 vs 609 + / - 56 IU/l , the peak CK-muscle-brain values , being 12 + / - 9 vs 16 + / - 5 IU/l , and the postoperative blood loss , being 369 + / - 198 vs 541 + / - 204 ml .
	manualset3
171706	3	413287	7	NULL	NULL	0	NULL	off-pump group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences between the MIDCAB group and the off-pump group in age , being 57 + / - 11 vs 66 + / - 8 years old , the operative time , being 321 + / - 149 vs 441 + / - 205 min , the number of grafts , being 1.0 vs 1.4 / patient , peak creatine kinase ( CK ) values , being 662 + / - 436 vs 609 + / - 56 IU/l , the peak CK-muscle-brain values , being 12 + / - 9 vs 16 + / - 5 IU/l , and the postoperative blood loss , being 369 + / - 198 vs 541 + / - 204 ml .
	manualset3
171707	4	413287	7	NULL	NULL	0	NULL	age	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences between the MIDCAB group and the off-pump group in age , being 57 + / - 11 vs 66 + / - 8 years old , the operative time , being 321 + / - 149 vs 441 + / - 205 min , the number of grafts , being 1.0 vs 1.4 / patient , peak creatine kinase ( CK ) values , being 662 + / - 436 vs 609 + / - 56 IU/l , the peak CK-muscle-brain values , being 12 + / - 9 vs 16 + / - 5 IU/l , and the postoperative blood loss , being 369 + / - 198 vs 541 + / - 204 ml .
	manualset3
171708	5	413287	7	NULL	NULL	0	NULL	57 + / - 11 years old	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences between the MIDCAB group and the off-pump group in age , being 57 + / - 11 vs 66 + / - 8 years old , the operative time , being 321 + / - 149 vs 441 + / - 205 min , the number of grafts , being 1.0 vs 1.4 / patient , peak creatine kinase ( CK ) values , being 662 + / - 436 vs 609 + / - 56 IU/l , the peak CK-muscle-brain values , being 12 + / - 9 vs 16 + / - 5 IU/l , and the postoperative blood loss , being 369 + / - 198 vs 541 + / - 204 ml .
	manualset3
171709	6	413287	7	NULL	NULL	0	NULL	66 + / - 8 years old	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences between the MIDCAB group and the off-pump group in age , being 57 + / - 11 vs 66 + / - 8 years old , the operative time , being 321 + / - 149 vs 441 + / - 205 min , the number of grafts , being 1.0 vs 1.4 / patient , peak creatine kinase ( CK ) values , being 662 + / - 436 vs 609 + / - 56 IU/l , the peak CK-muscle-brain values , being 12 + / - 9 vs 16 + / - 5 IU/l , and the postoperative blood loss , being 369 + / - 198 vs 541 + / - 204 ml .
	manualset3
171710	7	413287	7	NULL	NULL	0	NULL	operative time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences between the MIDCAB group and the off-pump group in age , being 57 + / - 11 vs 66 + / - 8 years old , the operative time , being 321 + / - 149 vs 441 + / - 205 min , the number of grafts , being 1.0 vs 1.4 / patient , peak creatine kinase ( CK ) values , being 662 + / - 436 vs 609 + / - 56 IU/l , the peak CK-muscle-brain values , being 12 + / - 9 vs 16 + / - 5 IU/l , and the postoperative blood loss , being 369 + / - 198 vs 541 + / - 204 ml .
	manualset3
171711	8	413287	7	NULL	NULL	0	NULL	321 + / - 149 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences between the MIDCAB group and the off-pump group in age , being 57 + / - 11 vs 66 + / - 8 years old , the operative time , being 321 + / - 149 vs 441 + / - 205 min , the number of grafts , being 1.0 vs 1.4 / patient , peak creatine kinase ( CK ) values , being 662 + / - 436 vs 609 + / - 56 IU/l , the peak CK-muscle-brain values , being 12 + / - 9 vs 16 + / - 5 IU/l , and the postoperative blood loss , being 369 + / - 198 vs 541 + / - 204 ml .
	manualset3
171712	9	413287	7	NULL	NULL	0	NULL	 441 + / - 205 min 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences between the MIDCAB group and the off-pump group in age , being 57 + / - 11 vs 66 + / - 8 years old , the operative time , being 321 + / - 149 vs 441 + / - 205 min , the number of grafts , being 1.0 vs 1.4 / patient , peak creatine kinase ( CK ) values , being 662 + / - 436 vs 609 + / - 56 IU/l , the peak CK-muscle-brain values , being 12 + / - 9 vs 16 + / - 5 IU/l , and the postoperative blood loss , being 369 + / - 198 vs 541 + / - 204 ml .
	manualset3
171713	10	413287	7	NULL	NULL	0	NULL	number of grafts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences between the MIDCAB group and the off-pump group in age , being 57 + / - 11 vs 66 + / - 8 years old , the operative time , being 321 + / - 149 vs 441 + / - 205 min , the number of grafts , being 1.0 vs 1.4 / patient , peak creatine kinase ( CK ) values , being 662 + / - 436 vs 609 + / - 56 IU/l , the peak CK-muscle-brain values , being 12 + / - 9 vs 16 + / - 5 IU/l , and the postoperative blood loss , being 369 + / - 198 vs 541 + / - 204 ml .
	manualset3
171714	11	413287	7	NULL	NULL	0	NULL	1.0 vs 1.4 / patient	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences between the MIDCAB group and the off-pump group in age , being 57 + / - 11 vs 66 + / - 8 years old , the operative time , being 321 + / - 149 vs 441 + / - 205 min , the number of grafts , being 1.0 vs 1.4 / patient , peak creatine kinase ( CK ) values , being 662 + / - 436 vs 609 + / - 56 IU/l , the peak CK-muscle-brain values , being 12 + / - 9 vs 16 + / - 5 IU/l , and the postoperative blood loss , being 369 + / - 198 vs 541 + / - 204 ml .
	manualset3
171715	12	413287	7	NULL	NULL	0	NULL	peak creatine kinase ( CK ) values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences between the MIDCAB group and the off-pump group in age , being 57 + / - 11 vs 66 + / - 8 years old , the operative time , being 321 + / - 149 vs 441 + / - 205 min , the number of grafts , being 1.0 vs 1.4 / patient , peak creatine kinase ( CK ) values , being 662 + / - 436 vs 609 + / - 56 IU/l , the peak CK-muscle-brain values , being 12 + / - 9 vs 16 + / - 5 IU/l , and the postoperative blood loss , being 369 + / - 198 vs 541 + / - 204 ml .
	manualset3
171716	13	413287	7	NULL	NULL	0	NULL	662 + / - 436	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences between the MIDCAB group and the off-pump group in age , being 57 + / - 11 vs 66 + / - 8 years old , the operative time , being 321 + / - 149 vs 441 + / - 205 min , the number of grafts , being 1.0 vs 1.4 / patient , peak creatine kinase ( CK ) values , being 662 + / - 436 vs 609 + / - 56 IU/l , the peak CK-muscle-brain values , being 12 + / - 9 vs 16 + / - 5 IU/l , and the postoperative blood loss , being 369 + / - 198 vs 541 + / - 204 ml .
	manualset3
171717	14	413287	7	NULL	NULL	NULL	NULL	609 + / - 56 IU/l	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There were no significant differences between the MIDCAB group and the off-pump group in age , being 57 + / - 11 vs 66 + / - 8 years old , the operative time , being 321 + / - 149 vs 441 + / - 205 min , the number of grafts , being 1.0 vs 1.4 / patient , peak creatine kinase ( CK ) values , being 662 + / - 436 vs 609 + / - 56 IU/l , the peak CK-muscle-brain values , being 12 + / - 9 vs 16 + / - 5 IU/l , and the postoperative blood loss , being 369 + / - 198 vs 541 + / - 204 ml .
	manualset3
171718	15	413287	7	NULL	NULL	0	NULL	peak CK-muscle-brain values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences between the MIDCAB group and the off-pump group in age , being 57 + / - 11 vs 66 + / - 8 years old , the operative time , being 321 + / - 149 vs 441 + / - 205 min , the number of grafts , being 1.0 vs 1.4 / patient , peak creatine kinase ( CK ) values , being 662 + / - 436 vs 609 + / - 56 IU/l , the peak CK-muscle-brain values , being 12 + / - 9 vs 16 + / - 5 IU/l , and the postoperative blood loss , being 369 + / - 198 vs 541 + / - 204 ml .
	manualset3
171719	16	413287	7	NULL	NULL	0	NULL	12 + / - 9	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences between the MIDCAB group and the off-pump group in age , being 57 + / - 11 vs 66 + / - 8 years old , the operative time , being 321 + / - 149 vs 441 + / - 205 min , the number of grafts , being 1.0 vs 1.4 / patient , peak creatine kinase ( CK ) values , being 662 + / - 436 vs 609 + / - 56 IU/l , the peak CK-muscle-brain values , being 12 + / - 9 vs 16 + / - 5 IU/l , and the postoperative blood loss , being 369 + / - 198 vs 541 + / - 204 ml .
	manualset3
171720	17	413287	7	NULL	NULL	0	NULL	16 + / - 5 IU/l	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences between the MIDCAB group and the off-pump group in age , being 57 + / - 11 vs 66 + / - 8 years old , the operative time , being 321 + / - 149 vs 441 + / - 205 min , the number of grafts , being 1.0 vs 1.4 / patient , peak creatine kinase ( CK ) values , being 662 + / - 436 vs 609 + / - 56 IU/l , the peak CK-muscle-brain values , being 12 + / - 9 vs 16 + / - 5 IU/l , and the postoperative blood loss , being 369 + / - 198 vs 541 + / - 204 ml .
	manualset3
171721	18	413287	7	NULL	NULL	0	NULL	postoperative blood loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences between the MIDCAB group and the off-pump group in age , being 57 + / - 11 vs 66 + / - 8 years old , the operative time , being 321 + / - 149 vs 441 + / - 205 min , the number of grafts , being 1.0 vs 1.4 / patient , peak creatine kinase ( CK ) values , being 662 + / - 436 vs 609 + / - 56 IU/l , the peak CK-muscle-brain values , being 12 + / - 9 vs 16 + / - 5 IU/l , and the postoperative blood loss , being 369 + / - 198 vs 541 + / - 204 ml .
	manualset3
171722	19	413287	7	NULL	NULL	0	NULL	369 + / - 198	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences between the MIDCAB group and the off-pump group in age , being 57 + / - 11 vs 66 + / - 8 years old , the operative time , being 321 + / - 149 vs 441 + / - 205 min , the number of grafts , being 1.0 vs 1.4 / patient , peak creatine kinase ( CK ) values , being 662 + / - 436 vs 609 + / - 56 IU/l , the peak CK-muscle-brain values , being 12 + / - 9 vs 16 + / - 5 IU/l , and the postoperative blood loss , being 369 + / - 198 vs 541 + / - 204 ml .
	manualset3
171723	20	413287	7	NULL	NULL	0	NULL	541 + / - 204 ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences between the MIDCAB group and the off-pump group in age , being 57 + / - 11 vs 66 + / - 8 years old , the operative time , being 321 + / - 149 vs 441 + / - 205 min , the number of grafts , being 1.0 vs 1.4 / patient , peak creatine kinase ( CK ) values , being 662 + / - 436 vs 609 + / - 56 IU/l , the peak CK-muscle-brain values , being 12 + / - 9 vs 16 + / - 5 IU/l , and the postoperative blood loss , being 369 + / - 198 vs 541 + / - 204 ml .
	manualset3
171724	1	413288	7	NULL	NULL	0	NULL	no significant differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences between the stevioside , rebaudioside A and no-addition groups .
	manualset3
171725	2	413288	7	NULL	NULL	0	NULL	stevioside	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences between the stevioside , rebaudioside A and no-addition groups .
	manualset3
171726	3	413288	7	NULL	NULL	0	NULL	rebaudioside A	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences between the stevioside , rebaudioside A and no-addition groups .
	manualset3
171727	4	413288	7	NULL	NULL	0	NULL	no-addition groups	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences between the stevioside , rebaudioside A and no-addition groups .
	manualset3
171728	1	413289	7	NULL	NULL	0	NULL	no significant differences 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences in the other metabolite increments ( alanine , lactate and pyruvate ; P ) / = 0.27 ) .
	manualset3
171729	2	413289	7	NULL	NULL	0	NULL	metabolite increments	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences in the other metabolite increments ( alanine , lactate and pyruvate ; P ) / = 0.27 ) .
	manualset3
171730	3	413289	7	NULL	NULL	0	NULL	alanine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences in the other metabolite increments ( alanine , lactate and pyruvate ; P ) / = 0.27 ) .
	manualset3
171731	4	413289	7	NULL	NULL	0	NULL	lactate	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences in the other metabolite increments ( alanine , lactate and pyruvate ; P ) / = 0.27 ) .
	manualset3
171732	5	413289	7	NULL	NULL	0	NULL	pyruvate	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences in the other metabolite increments ( alanine , lactate and pyruvate ; P ) / = 0.27 ) .
	manualset3
171733	6	413289	7	NULL	NULL	0	NULL	P  / = 0.27	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences in the other metabolite increments ( alanine , lactate and pyruvate ; P ) / = 0.27 ) .
	manualset3
171734	1	413290	7	NULL	NULL	0	NULL	no significant differences 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences in transplantation characteristics between the HLA DR15-positive and - negative groups .
	manualset3
171735	2	413290	7	NULL	NULL	0	NULL	transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences in transplantation characteristics between the HLA DR15-positive and - negative groups .
	manualset3
171736	3	413290	7	NULL	NULL	0	NULL	HLA DR15-positive groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences in transplantation characteristics between the HLA DR15-positive and - negative groups .
	manualset3
171737	4	413290	7	NULL	NULL	0	NULL	HLA DR15-negative groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences in transplantation characteristics between the HLA DR15-positive and - negative groups .
	manualset3
171738	1	413291	7	NULL	NULL	0	NULL	 no significant differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences in uptake or metabolism of radioactive testosterone among LA , MA , and HA males in homogenates of anterior and posterior hypothalamus , cerebral cortex , midbrain , or seminal vesicle .
	manualset3
171739	2	413291	7	NULL	NULL	0	NULL	uptake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences in uptake or metabolism of radioactive testosterone among LA , MA , and HA males in homogenates of anterior and posterior hypothalamus , cerebral cortex , midbrain , or seminal vesicle .
	manualset3
171740	3	413291	7	NULL	NULL	0	NULL	metabolism 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences in uptake or metabolism of radioactive testosterone among LA , MA , and HA males in homogenates of anterior and posterior hypothalamus , cerebral cortex , midbrain , or seminal vesicle .
	manualset3
171741	4	413291	7	NULL	NULL	0	NULL	radioactive testosterone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences in uptake or metabolism of radioactive testosterone among LA , MA , and HA males in homogenates of anterior and posterior hypothalamus , cerebral cortex , midbrain , or seminal vesicle .
	manualset3
171742	5	413291	7	NULL	NULL	0	NULL	 LA males	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences in uptake or metabolism of radioactive testosterone among LA , MA , and HA males in homogenates of anterior and posterior hypothalamus , cerebral cortex , midbrain , or seminal vesicle .
	manualset3
171743	6	413291	7	NULL	NULL	0	NULL	 MA males	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences in uptake or metabolism of radioactive testosterone among LA , MA , and HA males in homogenates of anterior and posterior hypothalamus , cerebral cortex , midbrain , or seminal vesicle .
	manualset3
171744	7	413291	7	NULL	NULL	0	NULL	HA males	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences in uptake or metabolism of radioactive testosterone among LA , MA , and HA males in homogenates of anterior and posterior hypothalamus , cerebral cortex , midbrain , or seminal vesicle .
	manualset3
171745	8	413291	7	NULL	NULL	0	NULL	homogenates	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences in uptake or metabolism of radioactive testosterone among LA , MA , and HA males in homogenates of anterior and posterior hypothalamus , cerebral cortex , midbrain , or seminal vesicle .
	manualset3
171746	9	413291	7	NULL	NULL	0	NULL	anterior and posterior hypothalamus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences in uptake or metabolism of radioactive testosterone among LA , MA , and HA males in homogenates of anterior and posterior hypothalamus , cerebral cortex , midbrain , or seminal vesicle .
	manualset3
171747	10	413291	7	NULL	NULL	0	NULL	cerebral cortex 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences in uptake or metabolism of radioactive testosterone among LA , MA , and HA males in homogenates of anterior and posterior hypothalamus , cerebral cortex , midbrain , or seminal vesicle .
	manualset3
171748	11	413291	7	NULL	NULL	0	NULL	midbrain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences in uptake or metabolism of radioactive testosterone among LA , MA , and HA males in homogenates of anterior and posterior hypothalamus , cerebral cortex , midbrain , or seminal vesicle .
	manualset3
171749	12	413291	7	NULL	NULL	0	NULL	seminal vesicle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no significant differences in uptake or metabolism of radioactive testosterone among LA , MA , and HA males in homogenates of anterior and posterior hypothalamus , cerebral cortex , midbrain , or seminal vesicle .
	manualset3
171750	1	413292	7	NULL	NULL	0	NULL	Activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity of selected rostral and caudal hyoid muscles in clinically normal horses during strenuous exercise .
	manualset3
171751	2	413292	7	NULL	NULL	0	NULL	selected rostral muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity of selected rostral and caudal hyoid muscles in clinically normal horses during strenuous exercise .
	manualset3
171752	3	413292	7	NULL	NULL	0	NULL	caudal hyoid muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity of selected rostral and caudal hyoid muscles in clinically normal horses during strenuous exercise .
	manualset3
171753	4	413292	7	NULL	NULL	0	NULL	 normal horses 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity of selected rostral and caudal hyoid muscles in clinically normal horses during strenuous exercise .
	manualset3
171754	5	413292	7	NULL	NULL	0	NULL	strenuous exercise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity of selected rostral and caudal hyoid muscles in clinically normal horses during strenuous exercise .
	manualset3
171755	1	413293	7	NULL	NULL	NULL	NULL	no study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There were no study about the effectiveness of physiotherapy in Hip-OA .
	manualset3
171756	2	413293	7	NULL	NULL	0	NULL	effectiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no study about the effectiveness of physiotherapy in Hip-OA .
	manualset3
171757	3	413293	7	NULL	NULL	0	NULL	physiotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no study about the effectiveness of physiotherapy in Hip-OA .
	manualset3
171758	4	413293	7	NULL	NULL	0	NULL	Hip-OA	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no study about the effectiveness of physiotherapy in Hip-OA .
	manualset3
171759	1	413294	7	NULL	NULL	0	NULL	significant morphological changes	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There were significant morphological changes , a higher cell growth inhibition rate and apoptosis rate and lesser expression of caspase-3 , 8 , 9 precursors in the cells treated with both cisplatin and DR5 ( D-6 ) .
	manualset3
171760	2	413294	7	NULL	NULL	0	NULL	higher cell growth inhibition rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There were significant morphological changes , a higher cell growth inhibition rate and apoptosis rate and lesser expression of caspase-3 , 8 , 9 precursors in the cells treated with both cisplatin and DR5 ( D-6 ) .
	manualset3
171761	3	413294	7	NULL	NULL	0	NULL	apoptosis rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There were significant morphological changes , a higher cell growth inhibition rate and apoptosis rate and lesser expression of caspase-3 , 8 , 9 precursors in the cells treated with both cisplatin and DR5 ( D-6 ) .
	manualset3
171762	4	413294	7	NULL	NULL	0	NULL	lesser expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There were significant morphological changes , a higher cell growth inhibition rate and apoptosis rate and lesser expression of caspase-3 , 8 , 9 precursors in the cells treated with both cisplatin and DR5 ( D-6 ) .
	manualset3
171763	5	413294	7	NULL	NULL	NULL	NULL	caspase-3 precursor	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There were significant morphological changes , a higher cell growth inhibition rate and apoptosis rate and lesser expression of caspase-3 , 8 , 9 precursors in the cells treated with both cisplatin and DR5 ( D-6 ) .
	manualset3
171764	6	413294	7	NULL	NULL	NULL	NULL	caspase-8 precursor	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There were significant morphological changes , a higher cell growth inhibition rate and apoptosis rate and lesser expression of caspase-3 , 8 , 9 precursors in the cells treated with both cisplatin and DR5 ( D-6 ) .
	manualset3
171765	7	413294	7	NULL	NULL	NULL	NULL	caspase-9 precursor	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There were significant morphological changes , a higher cell growth inhibition rate and apoptosis rate and lesser expression of caspase-3 , 8 , 9 precursors in the cells treated with both cisplatin and DR5 ( D-6 ) .
	manualset3
171766	8	413294	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	There were significant morphological changes , a higher cell growth inhibition rate and apoptosis rate and lesser expression of caspase-3 , 8 , 9 precursors in the cells treated with both cisplatin and DR5 ( D-6 ) .
	manualset3
171767	9	413294	7	NULL	NULL	0	NULL	cisplatin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	There were significant morphological changes , a higher cell growth inhibition rate and apoptosis rate and lesser expression of caspase-3 , 8 , 9 precursors in the cells treated with both cisplatin and DR5 ( D-6 ) .
	manualset3
171768	10	413294	7	NULL	NULL	0	NULL	DR5 ( D-6 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	There were significant morphological changes , a higher cell growth inhibition rate and apoptosis rate and lesser expression of caspase-3 , 8 , 9 precursors in the cells treated with both cisplatin and DR5 ( D-6 ) .
	manualset3
171769	1	413295	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There were slightly more women than men ( 53 % ) in the series .
	manualset3
171770	2	413295	7	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There were slightly more women than men ( 53 % ) in the series .
	manualset3
171771	3	413295	7	NULL	NULL	NULL	NULL	53 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There were slightly more women than men ( 53 % ) in the series .
	manualset3
171772	4	413295	7	NULL	NULL	0	NULL	series	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There were slightly more women than men ( 53 % ) in the series .
	manualset3
171773	1	413296	7	NULL	NULL	0	NULL	numbers of genes 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	There were substantial numbers of genes expressed more abundantly in ICC than in the tunica muscularis , and we also detected marked phenotypic differences between ICC-MY and ICC-DMP .
	manualset3
171774	2	413296	7	NULL	NULL	0	NULL	ICC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	There were substantial numbers of genes expressed more abundantly in ICC than in the tunica muscularis , and we also detected marked phenotypic differences between ICC-MY and ICC-DMP .
	manualset3
171775	3	413296	7	NULL	NULL	0	NULL	tunica muscularis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There were substantial numbers of genes expressed more abundantly in ICC than in the tunica muscularis , and we also detected marked phenotypic differences between ICC-MY and ICC-DMP .
	manualset3
171776	4	413296	7	NULL	NULL	0	NULL	marked phenotypic differences	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There were substantial numbers of genes expressed more abundantly in ICC than in the tunica muscularis , and we also detected marked phenotypic differences between ICC-MY and ICC-DMP .
	manualset3
171777	5	413296	7	NULL	NULL	0	NULL	ICC-MY	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There were substantial numbers of genes expressed more abundantly in ICC than in the tunica muscularis , and we also detected marked phenotypic differences between ICC-MY and ICC-DMP .
	manualset3
171778	6	413296	7	NULL	NULL	0	NULL	ICC-DMP	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There were substantial numbers of genes expressed more abundantly in ICC than in the tunica muscularis , and we also detected marked phenotypic differences between ICC-MY and ICC-DMP .
	manualset3
171779	1	413297	7	NULL	NULL	0	NULL	CNS	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There appears to be nothing unique about the manner in which the CNS responds to inflammation or in the molecules expressed .
	manualset3
171780	2	413297	7	NULL	NULL	0	NULL	 inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There appears to be nothing unique about the manner in which the CNS responds to inflammation or in the molecules expressed .
	manualset3
171781	3	413297	7	NULL	NULL	0	NULL	molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	There appears to be nothing unique about the manner in which the CNS responds to inflammation or in the molecules expressed .
	manualset3
171782	1	413298	7	NULL	NULL	0	NULL	Activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity of these tannin preparations tracks to the procyanidin fraction , with the procyanidin trimer ( C1 ) having the most robust activity defined to date .
	manualset3
171783	2	413298	7	NULL	NULL	0	NULL	tannin preparations	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity of these tannin preparations tracks to the procyanidin fraction , with the procyanidin trimer ( C1 ) having the most robust activity defined to date .
	manualset3
171784	3	413298	7	NULL	NULL	0	NULL	 procyanidin fraction	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity of these tannin preparations tracks to the procyanidin fraction , with the procyanidin trimer ( C1 ) having the most robust activity defined to date .
	manualset3
171785	4	413298	7	NULL	NULL	0	NULL	procyanidin trimer ( C1 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity of these tannin preparations tracks to the procyanidin fraction , with the procyanidin trimer ( C1 ) having the most robust activity defined to date .
	manualset3
171786	5	413298	7	NULL	NULL	0	NULL	activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity of these tannin preparations tracks to the procyanidin fraction , with the procyanidin trimer ( C1 ) having the most robust activity defined to date .
	manualset3
171787	1	413299	7	NULL	NULL	0	NULL	 influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There appears to have been little influence of the MUC on the curricula of military family practice residencies since its publication .
	manualset3
171788	2	413299	7	NULL	NULL	0	NULL	 MUC	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There appears to have been little influence of the MUC on the curricula of military family practice residencies since its publication .
	manualset3
171789	3	413299	7	NULL	NULL	0	NULL	curricula	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	There appears to have been little influence of the MUC on the curricula of military family practice residencies since its publication .
	manualset3
171790	4	413299	7	NULL	NULL	0	NULL	military family practice residencies	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	There appears to have been little influence of the MUC on the curricula of military family practice residencies since its publication .
	manualset3
171791	5	413299	7	NULL	NULL	0	NULL	publication	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	There appears to have been little influence of the MUC on the curricula of military family practice residencies since its publication .
	manualset3
171792	1	413300	7	NULL	NULL	0	NULL	Ca2 + - induced Pyk2/Src complex formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , Ca2 + - induced Pyk2/Src complex formation may be a rewarding molecular target for novel therapeutic strategies in SCLC cells .
	manualset3
171793	2	413300	7	NULL	NULL	0	NULL	molecular target	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , Ca2 + - induced Pyk2/Src complex formation may be a rewarding molecular target for novel therapeutic strategies in SCLC cells .
	manualset3
171794	3	413300	7	NULL	NULL	0	NULL	novel therapeutic strategies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , Ca2 + - induced Pyk2/Src complex formation may be a rewarding molecular target for novel therapeutic strategies in SCLC cells .
	manualset3
171795	4	413300	7	NULL	NULL	0	NULL	SCLC cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , Ca2 + - induced Pyk2/Src complex formation may be a rewarding molecular target for novel therapeutic strategies in SCLC cells .
	manualset3
171796	1	413301	7	NULL	NULL	0	NULL	Hox gene patterning activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , Hox gene patterning activity is different in the somites and presomitic mesoderm , the latter being very prominent for Hox gene-mediated patterning of the axial skeleton .
	manualset3
171797	2	413301	7	NULL	NULL	0	NULL	somites	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , Hox gene patterning activity is different in the somites and presomitic mesoderm , the latter being very prominent for Hox gene-mediated patterning of the axial skeleton .
	manualset3
171798	3	413301	7	NULL	NULL	0	NULL	presomitic mesoderm	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , Hox gene patterning activity is different in the somites and presomitic mesoderm , the latter being very prominent for Hox gene-mediated patterning of the axial skeleton .
	manualset3
171799	4	413301	7	NULL	NULL	0	NULL	Hox gene-mediated patterning	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , Hox gene patterning activity is different in the somites and presomitic mesoderm , the latter being very prominent for Hox gene-mediated patterning of the axial skeleton .
	manualset3
171800	5	413301	7	NULL	NULL	0	NULL	axial skeleton	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , Hox gene patterning activity is different in the somites and presomitic mesoderm , the latter being very prominent for Hox gene-mediated patterning of the axial skeleton .
	manualset3
171801	1	413302	7	NULL	NULL	0	NULL	OX40	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , OX40 primarily functions to augment PKB signaling in T cells by enhancing the amount of PI3K and PKB available to the TCR .
	manualset3
171802	2	413302	7	NULL	NULL	0	NULL	PKB signaling 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , OX40 primarily functions to augment PKB signaling in T cells by enhancing the amount of PI3K and PKB available to the TCR .
	manualset3
171803	3	413302	7	NULL	NULL	0	NULL	T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , OX40 primarily functions to augment PKB signaling in T cells by enhancing the amount of PI3K and PKB available to the TCR .
	manualset3
171804	4	413302	7	NULL	NULL	0	NULL	enhancing	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , OX40 primarily functions to augment PKB signaling in T cells by enhancing the amount of PI3K and PKB available to the TCR .
	manualset3
171805	5	413302	7	NULL	NULL	0	NULL	 amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , OX40 primarily functions to augment PKB signaling in T cells by enhancing the amount of PI3K and PKB available to the TCR .
	manualset3
171806	6	413302	7	NULL	NULL	0	NULL	PI3K	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , OX40 primarily functions to augment PKB signaling in T cells by enhancing the amount of PI3K and PKB available to the TCR .
	manualset3
171807	7	413302	7	NULL	NULL	0	NULL	PKB	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , OX40 primarily functions to augment PKB signaling in T cells by enhancing the amount of PI3K and PKB available to the TCR .
	manualset3
171808	8	413302	7	NULL	NULL	0	NULL	TCR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , OX40 primarily functions to augment PKB signaling in T cells by enhancing the amount of PI3K and PKB available to the TCR .
	manualset3
171809	1	413303	7	NULL	NULL	0	NULL	PCI	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , PCI , duration of heparin treatment and thrombotic history facilitated the seroconversion in ACS patients .
	manualset3
171810	2	413303	7	NULL	NULL	0	NULL	duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , PCI , duration of heparin treatment and thrombotic history facilitated the seroconversion in ACS patients .
	manualset3
171811	3	413303	7	NULL	NULL	NULL	NULL	 heparin treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , PCI , duration of heparin treatment and thrombotic history facilitated the seroconversion in ACS patients .
	manualset3
171812	4	413303	7	NULL	NULL	0	NULL	thrombotic history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , PCI , duration of heparin treatment and thrombotic history facilitated the seroconversion in ACS patients .
	manualset3
171813	5	413303	7	NULL	NULL	0	NULL	seroconversion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , PCI , duration of heparin treatment and thrombotic history facilitated the seroconversion in ACS patients .
	manualset3
171814	6	413303	7	NULL	NULL	0	NULL	ACS patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , PCI , duration of heparin treatment and thrombotic history facilitated the seroconversion in ACS patients .
	manualset3
171815	1	413304	7	NULL	NULL	0	NULL	Spodoptera frugiperda ( Sf9 ) cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , Spodoptera frugiperda ( Sf9 ) cells and baculovirus have been evaluated for high-level and functional expression of AhR .
	manualset3
171816	2	413304	7	NULL	NULL	0	NULL	baculovirus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , Spodoptera frugiperda ( Sf9 ) cells and baculovirus have been evaluated for high-level and functional expression of AhR .
	manualset3
171817	3	413304	7	NULL	NULL	0	NULL	high-level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , Spodoptera frugiperda ( Sf9 ) cells and baculovirus have been evaluated for high-level and functional expression of AhR .
	manualset3
171818	4	413304	7	NULL	NULL	0	NULL	 functional expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , Spodoptera frugiperda ( Sf9 ) cells and baculovirus have been evaluated for high-level and functional expression of AhR .
	manualset3
171819	5	413304	7	NULL	NULL	0	NULL	 AhR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , Spodoptera frugiperda ( Sf9 ) cells and baculovirus have been evaluated for high-level and functional expression of AhR .
	manualset3
171820	1	413305	7	NULL	NULL	NULL	NULL	depression	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , a depression of KI with elevation of SOP of PMN may serve to predict complications of infection following surgery in patients with esophageal cancer .
	manualset3
171821	2	413305	7	NULL	NULL	0	NULL	KI	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , a depression of KI with elevation of SOP of PMN may serve to predict complications of infection following surgery in patients with esophageal cancer .
	manualset3
171822	3	413305	7	NULL	NULL	0	NULL	elevation	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , a depression of KI with elevation of SOP of PMN may serve to predict complications of infection following surgery in patients with esophageal cancer .
	manualset3
171823	4	413305	7	NULL	NULL	0	NULL	SOP	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , a depression of KI with elevation of SOP of PMN may serve to predict complications of infection following surgery in patients with esophageal cancer .
	manualset3
171824	5	413305	7	NULL	NULL	0	NULL	 PMN	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , a depression of KI with elevation of SOP of PMN may serve to predict complications of infection following surgery in patients with esophageal cancer .
	manualset3
171825	6	413305	7	NULL	NULL	0	NULL	complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , a depression of KI with elevation of SOP of PMN may serve to predict complications of infection following surgery in patients with esophageal cancer .
	manualset3
171826	7	413305	7	NULL	NULL	0	NULL	infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , a depression of KI with elevation of SOP of PMN may serve to predict complications of infection following surgery in patients with esophageal cancer .
	manualset3
171827	8	413305	7	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , a depression of KI with elevation of SOP of PMN may serve to predict complications of infection following surgery in patients with esophageal cancer .
	manualset3
171828	9	413305	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , a depression of KI with elevation of SOP of PMN may serve to predict complications of infection following surgery in patients with esophageal cancer .
	manualset3
171829	10	413305	7	NULL	NULL	0	NULL	esophageal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , a depression of KI with elevation of SOP of PMN may serve to predict complications of infection following surgery in patients with esophageal cancer .
	manualset3
171830	1	413306	7	NULL	NULL	0	NULL	Comparative analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative analysis of two diffusion methods for radon Rn-222 estimation in atmospheric air by means of gamma ray spectrometry and liquid scintillation counting ) .
	manualset3
171831	2	413306	7	NULL	NULL	0	NULL	two diffusion methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative analysis of two diffusion methods for radon Rn-222 estimation in atmospheric air by means of gamma ray spectrometry and liquid scintillation counting ) .
	manualset3
171832	3	413306	7	NULL	NULL	NULL	NULL	radon Rn-222 estimation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Comparative analysis of two diffusion methods for radon Rn-222 estimation in atmospheric air by means of gamma ray spectrometry and liquid scintillation counting ) .
	manualset3
171833	4	413306	7	NULL	NULL	0	NULL	atmospheric air	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative analysis of two diffusion methods for radon Rn-222 estimation in atmospheric air by means of gamma ray spectrometry and liquid scintillation counting ) .
	manualset3
171834	5	413306	7	NULL	NULL	0	NULL	 gamma ray spectrometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative analysis of two diffusion methods for radon Rn-222 estimation in atmospheric air by means of gamma ray spectrometry and liquid scintillation counting ) .
	manualset3
171835	6	413306	7	NULL	NULL	0	NULL	liquid scintillation counting	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative analysis of two diffusion methods for radon Rn-222 estimation in atmospheric air by means of gamma ray spectrometry and liquid scintillation counting ) .
	manualset3
171836	1	413307	7	NULL	NULL	0	NULL	Actuarial risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Actuarial risk of MF was as low as 4.9 and 9.4 % at 10 and 15 years , respectively .
	manualset3
171837	2	413307	7	NULL	NULL	0	NULL	 MF	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Actuarial risk of MF was as low as 4.9 and 9.4 % at 10 and 15 years , respectively .
	manualset3
171838	3	413307	7	NULL	NULL	0	NULL	4.9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Actuarial risk of MF was as low as 4.9 and 9.4 % at 10 and 15 years , respectively .
	manualset3
171839	4	413307	7	NULL	NULL	0	NULL	9.4 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Actuarial risk of MF was as low as 4.9 and 9.4 % at 10 and 15 years , respectively .
	manualset3
171840	5	413307	7	NULL	NULL	0	NULL	10 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Actuarial risk of MF was as low as 4.9 and 9.4 % at 10 and 15 years , respectively .
	manualset3
171841	6	413307	7	NULL	NULL	0	NULL	15 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Actuarial risk of MF was as low as 4.9 and 9.4 % at 10 and 15 years , respectively .
	manualset3
171842	1	413308	7	NULL	NULL	NULL	NULL	meta-analysis	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , a meta-analysis of randomized trials was performed to compare SES with PES exclusively in patients with diabetes .
	manualset3
171843	2	413308	7	NULL	NULL	0	NULL	 randomized trials 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , a meta-analysis of randomized trials was performed to compare SES with PES exclusively in patients with diabetes .
	manualset3
171844	3	413308	7	NULL	NULL	0	NULL	SES	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , a meta-analysis of randomized trials was performed to compare SES with PES exclusively in patients with diabetes .
	manualset3
171845	4	413308	7	NULL	NULL	0	NULL	 PES	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , a meta-analysis of randomized trials was performed to compare SES with PES exclusively in patients with diabetes .
	manualset3
171846	5	413308	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , a meta-analysis of randomized trials was performed to compare SES with PES exclusively in patients with diabetes .
	manualset3
171847	6	413308	7	NULL	NULL	0	NULL	diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , a meta-analysis of randomized trials was performed to compare SES with PES exclusively in patients with diabetes .
	manualset3
171848	1	413309	7	NULL	NULL	0	NULL	substantial portion	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , a substantial portion of the TF surface ( 3000 A ( 2 ) ) is engaged in protein-protein interactions during substrate catalysis .
	manualset3
171849	2	413309	7	NULL	NULL	0	NULL	TF surface	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , a substantial portion of the TF surface ( 3000 A ( 2 ) ) is engaged in protein-protein interactions during substrate catalysis .
	manualset3
171850	3	413309	7	NULL	NULL	0	NULL	( 3000 A ( 2 ) )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , a substantial portion of the TF surface ( 3000 A ( 2 ) ) is engaged in protein-protein interactions during substrate catalysis .
	manualset3
171851	4	413309	7	NULL	NULL	0	NULL	protein-protein interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , a substantial portion of the TF surface ( 3000 A ( 2 ) ) is engaged in protein-protein interactions during substrate catalysis .
	manualset3
171852	5	413309	7	NULL	NULL	0	NULL	substrate catalysis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , a substantial portion of the TF surface ( 3000 A ( 2 ) ) is engaged in protein-protein interactions during substrate catalysis .
	manualset3
171853	1	413310	7	NULL	NULL	0	NULL	control mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , additional control mechanisms , involving higher ATPase flux and ( Ca2 + ) , must exist to explain the well-known difference in glycolytic rates in fast-twitch and slow-twitch muscles in actively contracting muscle .
	manualset3
171854	2	413310	7	NULL	NULL	0	NULL	higher ATPase flux	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , additional control mechanisms , involving higher ATPase flux and ( Ca2 + ) , must exist to explain the well-known difference in glycolytic rates in fast-twitch and slow-twitch muscles in actively contracting muscle .
	manualset3
171855	3	413310	7	NULL	NULL	0	NULL	Ca2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , additional control mechanisms , involving higher ATPase flux and ( Ca2 + ) , must exist to explain the well-known difference in glycolytic rates in fast-twitch and slow-twitch muscles in actively contracting muscle .
	manualset3
171856	4	413310	7	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , additional control mechanisms , involving higher ATPase flux and ( Ca2 + ) , must exist to explain the well-known difference in glycolytic rates in fast-twitch and slow-twitch muscles in actively contracting muscle .
	manualset3
171857	5	413310	7	NULL	NULL	0	NULL	glycolytic rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , additional control mechanisms , involving higher ATPase flux and ( Ca2 + ) , must exist to explain the well-known difference in glycolytic rates in fast-twitch and slow-twitch muscles in actively contracting muscle .
	manualset3
171858	6	413310	7	NULL	NULL	0	NULL	fast-twitch muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , additional control mechanisms , involving higher ATPase flux and ( Ca2 + ) , must exist to explain the well-known difference in glycolytic rates in fast-twitch and slow-twitch muscles in actively contracting muscle .
	manualset3
171859	7	413310	7	NULL	NULL	0	NULL	slow-twitch muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , additional control mechanisms , involving higher ATPase flux and ( Ca2 + ) , must exist to explain the well-known difference in glycolytic rates in fast-twitch and slow-twitch muscles in actively contracting muscle .
	manualset3
171860	8	413310	7	NULL	NULL	0	NULL	actively contracting muscle	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , additional control mechanisms , involving higher ATPase flux and ( Ca2 + ) , must exist to explain the well-known difference in glycolytic rates in fast-twitch and slow-twitch muscles in actively contracting muscle .
	manualset3
171861	1	413311	7	NULL	NULL	0	NULL	beta 2-agonists	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , beta 2-agonists may prove useful in prevention and/or treatment of cancer cachexia .
	manualset3
171862	2	413311	7	NULL	NULL	0	NULL	prevention 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , beta 2-agonists may prove useful in prevention and/or treatment of cancer cachexia .
	manualset3
171863	3	413311	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , beta 2-agonists may prove useful in prevention and/or treatment of cancer cachexia .
	manualset3
171864	4	413311	7	NULL	NULL	0	NULL	cancer cachexia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , beta 2-agonists may prove useful in prevention and/or treatment of cancer cachexia .
	manualset3
171865	1	413312	7	NULL	NULL	0	NULL	cardioprotective mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , cardioprotective mechanisms both dependent and independent of SUR2-K ( ATP ) channels contribute to cardiac function .
	manualset3
171866	2	413312	7	NULL	NULL	0	NULL	SUR2-K ( ATP ) channels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , cardioprotective mechanisms both dependent and independent of SUR2-K ( ATP ) channels contribute to cardiac function .
	manualset3
171867	3	413312	7	NULL	NULL	0	NULL	 cardiac function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , cardioprotective mechanisms both dependent and independent of SUR2-K ( ATP ) channels contribute to cardiac function .
	manualset3
171868	1	413313	7	NULL	NULL	0	NULL	cardiovascular responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , cardiovascular and adrenal responses to mental stress were abnormally high in subjects with hyperthyroidism .
	manualset3
171869	2	413313	7	NULL	NULL	0	NULL	adrenal responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , cardiovascular and adrenal responses to mental stress were abnormally high in subjects with hyperthyroidism .
	manualset3
171870	3	413313	7	NULL	NULL	0	NULL	mental stress 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , cardiovascular and adrenal responses to mental stress were abnormally high in subjects with hyperthyroidism .
	manualset3
171871	4	413313	7	NULL	NULL	0	NULL	high	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , cardiovascular and adrenal responses to mental stress were abnormally high in subjects with hyperthyroidism .
	manualset3
171872	5	413313	7	NULL	NULL	0	NULL	subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , cardiovascular and adrenal responses to mental stress were abnormally high in subjects with hyperthyroidism .
	manualset3
171873	6	413313	7	NULL	NULL	0	NULL	hyperthyroidism	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , cardiovascular and adrenal responses to mental stress were abnormally high in subjects with hyperthyroidism .
	manualset3
171874	1	413314	7	NULL	NULL	0	NULL	consideration 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , careful consideration should be given to the possibility that lung inflammation or fibrosis could be significant side effects caused by a CNT-based drug-delivery system , thereby outweighing any potential beneficial effects of therapeutic treatment .
	manualset3
171875	2	413314	7	NULL	NULL	0	NULL	possibility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , careful consideration should be given to the possibility that lung inflammation or fibrosis could be significant side effects caused by a CNT-based drug-delivery system , thereby outweighing any potential beneficial effects of therapeutic treatment .
	manualset3
171876	3	413314	7	NULL	NULL	0	NULL	lung inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , careful consideration should be given to the possibility that lung inflammation or fibrosis could be significant side effects caused by a CNT-based drug-delivery system , thereby outweighing any potential beneficial effects of therapeutic treatment .
	manualset3
171877	4	413314	7	NULL	NULL	0	NULL	 fibrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , careful consideration should be given to the possibility that lung inflammation or fibrosis could be significant side effects caused by a CNT-based drug-delivery system , thereby outweighing any potential beneficial effects of therapeutic treatment .
	manualset3
171878	5	413314	7	NULL	NULL	0	NULL	side effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , careful consideration should be given to the possibility that lung inflammation or fibrosis could be significant side effects caused by a CNT-based drug-delivery system , thereby outweighing any potential beneficial effects of therapeutic treatment .
	manualset3
171879	6	413314	7	NULL	NULL	0	NULL	CNT-based drug-delivery system	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , careful consideration should be given to the possibility that lung inflammation or fibrosis could be significant side effects caused by a CNT-based drug-delivery system , thereby outweighing any potential beneficial effects of therapeutic treatment .
	manualset3
171880	7	413314	7	NULL	NULL	0	NULL	outweighing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , careful consideration should be given to the possibility that lung inflammation or fibrosis could be significant side effects caused by a CNT-based drug-delivery system , thereby outweighing any potential beneficial effects of therapeutic treatment .
	manualset3
171881	8	413314	7	NULL	NULL	0	NULL	 beneficial effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , careful consideration should be given to the possibility that lung inflammation or fibrosis could be significant side effects caused by a CNT-based drug-delivery system , thereby outweighing any potential beneficial effects of therapeutic treatment .
	manualset3
171882	9	413314	7	NULL	NULL	0	NULL	therapeutic treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , careful consideration should be given to the possibility that lung inflammation or fibrosis could be significant side effects caused by a CNT-based drug-delivery system , thereby outweighing any potential beneficial effects of therapeutic treatment .
	manualset3
171883	1	413315	7	NULL	NULL	0	NULL	chemisorption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , chemisorption and physisorption coexisted during phosphate adsorption onto FHMD .
	manualset3
171884	2	413315	7	NULL	NULL	0	NULL	physisorption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , chemisorption and physisorption coexisted during phosphate adsorption onto FHMD .
	manualset3
171885	3	413315	7	NULL	NULL	0	NULL	phosphate adsorption 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , chemisorption and physisorption coexisted during phosphate adsorption onto FHMD .
	manualset3
171886	4	413315	7	NULL	NULL	0	NULL	FHMD	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , chemisorption and physisorption coexisted during phosphate adsorption onto FHMD .
	manualset3
171887	1	413316	7	NULL	NULL	0	NULL	deletion or altered regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , deletion or altered regulation of p16INK4a and p15INK4b occur concomitantly with the loss of differentiation associated with the late spindle stage of tumor progression in mouse skin .
	manualset3
171888	2	413316	7	NULL	NULL	0	NULL	p16INK4a	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , deletion or altered regulation of p16INK4a and p15INK4b occur concomitantly with the loss of differentiation associated with the late spindle stage of tumor progression in mouse skin .
	manualset3
171889	3	413316	7	NULL	NULL	0	NULL	p15INK4b	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , deletion or altered regulation of p16INK4a and p15INK4b occur concomitantly with the loss of differentiation associated with the late spindle stage of tumor progression in mouse skin .
	manualset3
171890	4	413316	7	NULL	NULL	NULL	NULL	loss of differentiation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , deletion or altered regulation of p16INK4a and p15INK4b occur concomitantly with the loss of differentiation associated with the late spindle stage of tumor progression in mouse skin .
	manualset3
171892	6	413316	7	NULL	NULL	0	NULL	late spindle stage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , deletion or altered regulation of p16INK4a and p15INK4b occur concomitantly with the loss of differentiation associated with the late spindle stage of tumor progression in mouse skin .
	manualset3
171893	7	413316	7	NULL	NULL	0	NULL	tumor progression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , deletion or altered regulation of p16INK4a and p15INK4b occur concomitantly with the loss of differentiation associated with the late spindle stage of tumor progression in mouse skin .
	manualset3
171894	8	413316	7	NULL	NULL	0	NULL	mouse skin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , deletion or altered regulation of p16INK4a and p15INK4b occur concomitantly with the loss of differentiation associated with the late spindle stage of tumor progression in mouse skin .
	manualset3
171895	1	413317	7	NULL	NULL	0	NULL	early detection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , early detection , prompt treatment , discontinuation of triggering agents , and sufficient administration of dantrolene are needed .
	manualset3
171896	2	413317	7	NULL	NULL	0	NULL	prompt treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , early detection , prompt treatment , discontinuation of triggering agents , and sufficient administration of dantrolene are needed .
	manualset3
171897	3	413317	7	NULL	NULL	NULL	NULL	discontinuation of triggering agents	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , early detection , prompt treatment , discontinuation of triggering agents , and sufficient administration of dantrolene are needed .
	manualset3
171898	4	413317	7	NULL	NULL	0	NULL	administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , early detection , prompt treatment , discontinuation of triggering agents , and sufficient administration of dantrolene are needed .
	manualset3
171899	5	413317	7	NULL	NULL	0	NULL	dantrolene	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , early detection , prompt treatment , discontinuation of triggering agents , and sufficient administration of dantrolene are needed .
	manualset3
171900	1	413318	7	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , further research is needed in the fields of epidemiology and epizootiology .
	manualset3
171901	2	413318	7	NULL	NULL	0	NULL	fields	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , further research is needed in the fields of epidemiology and epizootiology .
	manualset3
171902	3	413318	7	NULL	NULL	0	NULL	epidemiology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , further research is needed in the fields of epidemiology and epizootiology .
	manualset3
171903	4	413318	7	NULL	NULL	0	NULL	epizootiology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , further research is needed in the fields of epidemiology and epizootiology .
	manualset3
171904	1	413319	7	NULL	NULL	0	NULL	hypothermia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , hypothermia spares cardiac glycogen during asphyxia , but there are factors other than cardiac glycogen which influence survival of asphyxiated animals .
	manualset3
171905	2	413319	7	NULL	NULL	0	NULL	 cardiac glycogen	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , hypothermia spares cardiac glycogen during asphyxia , but there are factors other than cardiac glycogen which influence survival of asphyxiated animals .
	manualset3
171906	3	413319	7	NULL	NULL	0	NULL	asphyxia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , hypothermia spares cardiac glycogen during asphyxia , but there are factors other than cardiac glycogen which influence survival of asphyxiated animals .
	manualset3
171907	4	413319	7	NULL	NULL	0	NULL	 factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , hypothermia spares cardiac glycogen during asphyxia , but there are factors other than cardiac glycogen which influence survival of asphyxiated animals .
	manualset3
171908	5	413319	7	NULL	NULL	0	NULL	cardiac glycogen	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , hypothermia spares cardiac glycogen during asphyxia , but there are factors other than cardiac glycogen which influence survival of asphyxiated animals .
	manualset3
171909	6	413319	7	NULL	NULL	0	NULL	survival 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , hypothermia spares cardiac glycogen during asphyxia , but there are factors other than cardiac glycogen which influence survival of asphyxiated animals .
	manualset3
171910	7	413319	7	NULL	NULL	0	NULL	asphyxiated animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , hypothermia spares cardiac glycogen during asphyxia , but there are factors other than cardiac glycogen which influence survival of asphyxiated animals .
	manualset3
171912	1	413320	7	NULL	NULL	NULL	NULL	 view	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , in view of the lack of selective purinergic agonists and antagonists , we used P2Y2-deficient mice to clarify the action of UTP .
	manualset3
171913	2	413320	7	NULL	NULL	0	NULL	 lack	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , in view of the lack of selective purinergic agonists and antagonists , we used P2Y2-deficient mice to clarify the action of UTP .
	manualset3
171914	3	413320	7	NULL	NULL	0	NULL	 selective purinergic agonists	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , in view of the lack of selective purinergic agonists and antagonists , we used P2Y2-deficient mice to clarify the action of UTP .
	manualset3
171915	4	413320	7	NULL	NULL	0	NULL	selective purinergic antagonists	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , in view of the lack of selective purinergic agonists and antagonists , we used P2Y2-deficient mice to clarify the action of UTP .
	manualset3
171916	5	413320	7	NULL	NULL	0	NULL	P2Y2-deficient mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , in view of the lack of selective purinergic agonists and antagonists , we used P2Y2-deficient mice to clarify the action of UTP .
	manualset3
171917	6	413320	7	NULL	NULL	0	NULL	action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , in view of the lack of selective purinergic agonists and antagonists , we used P2Y2-deficient mice to clarify the action of UTP .
	manualset3
171918	7	413320	7	NULL	NULL	0	NULL	UTP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , in view of the lack of selective purinergic agonists and antagonists , we used P2Y2-deficient mice to clarify the action of UTP .
	manualset3
171919	1	413321	7	NULL	NULL	0	NULL	inclusion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , inclusion of new functional ingredients to pediatric milk formulas is , nowadays , the matter of a number of studies , incorporating day-by-day newer products and more similar to human milk , the gold standard , which contains them in a natural way .
	manualset3
171920	2	413321	7	NULL	NULL	0	NULL	new functional ingredients	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , inclusion of new functional ingredients to pediatric milk formulas is , nowadays , the matter of a number of studies , incorporating day-by-day newer products and more similar to human milk , the gold standard , which contains them in a natural way .
	manualset3
171921	3	413321	7	NULL	NULL	0	NULL	pediatric milk formulas	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , inclusion of new functional ingredients to pediatric milk formulas is , nowadays , the matter of a number of studies , incorporating day-by-day newer products and more similar to human milk , the gold standard , which contains them in a natural way .
	manualset3
171922	4	413321	7	NULL	NULL	0	NULL	nowadays	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , inclusion of new functional ingredients to pediatric milk formulas is , nowadays , the matter of a number of studies , incorporating day-by-day newer products and more similar to human milk , the gold standard , which contains them in a natural way .
	manualset3
171923	5	413321	7	NULL	NULL	0	NULL	matter	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , inclusion of new functional ingredients to pediatric milk formulas is , nowadays , the matter of a number of studies , incorporating day-by-day newer products and more similar to human milk , the gold standard , which contains them in a natural way .
	manualset3
171924	6	413321	7	NULL	NULL	0	NULL	number of studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , inclusion of new functional ingredients to pediatric milk formulas is , nowadays , the matter of a number of studies , incorporating day-by-day newer products and more similar to human milk , the gold standard , which contains them in a natural way .
	manualset3
171925	7	413321	7	NULL	NULL	0	NULL	day-by-day newer products	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , inclusion of new functional ingredients to pediatric milk formulas is , nowadays , the matter of a number of studies , incorporating day-by-day newer products and more similar to human milk , the gold standard , which contains them in a natural way .
	manualset3
171926	8	413321	7	NULL	NULL	0	NULL	similar	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , inclusion of new functional ingredients to pediatric milk formulas is , nowadays , the matter of a number of studies , incorporating day-by-day newer products and more similar to human milk , the gold standard , which contains them in a natural way .
	manualset3
171927	9	413321	7	NULL	NULL	0	NULL	human milk	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , inclusion of new functional ingredients to pediatric milk formulas is , nowadays , the matter of a number of studies , incorporating day-by-day newer products and more similar to human milk , the gold standard , which contains them in a natural way .
	manualset3
171928	10	413321	7	NULL	NULL	0	NULL	gold standard	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , inclusion of new functional ingredients to pediatric milk formulas is , nowadays , the matter of a number of studies , incorporating day-by-day newer products and more similar to human milk , the gold standard , which contains them in a natural way .
	manualset3
171929	11	413321	7	NULL	NULL	0	NULL	natural way	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , inclusion of new functional ingredients to pediatric milk formulas is , nowadays , the matter of a number of studies , incorporating day-by-day newer products and more similar to human milk , the gold standard , which contains them in a natural way .
	manualset3
171930	1	413322	7	NULL	NULL	0	NULL	Actuarial survivals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Actuarial survivals at 8 years were 68 % , 44 % , and 15 % , respectively ( p less than .01 ) , with 1 to 165 months of follow-up ( mean 52 ) .
	manualset3
171931	2	413322	7	NULL	NULL	0	NULL	8 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Actuarial survivals at 8 years were 68 % , 44 % , and 15 % , respectively ( p less than .01 ) , with 1 to 165 months of follow-up ( mean 52 ) .
	manualset3
171932	3	413322	7	NULL	NULL	0	NULL	 68 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Actuarial survivals at 8 years were 68 % , 44 % , and 15 % , respectively ( p less than .01 ) , with 1 to 165 months of follow-up ( mean 52 ) .
	manualset3
171933	4	413322	7	NULL	NULL	0	NULL	44 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Actuarial survivals at 8 years were 68 % , 44 % , and 15 % , respectively ( p less than .01 ) , with 1 to 165 months of follow-up ( mean 52 ) .
	manualset3
171934	5	413322	7	NULL	NULL	0	NULL	15 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Actuarial survivals at 8 years were 68 % , 44 % , and 15 % , respectively ( p less than .01 ) , with 1 to 165 months of follow-up ( mean 52 ) .
	manualset3
171935	6	413322	7	NULL	NULL	0	NULL	 p less than .01	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Actuarial survivals at 8 years were 68 % , 44 % , and 15 % , respectively ( p less than .01 ) , with 1 to 165 months of follow-up ( mean 52 ) .
	manualset3
171936	7	413322	7	NULL	NULL	0	NULL	1 to 165 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Actuarial survivals at 8 years were 68 % , 44 % , and 15 % , respectively ( p less than .01 ) , with 1 to 165 months of follow-up ( mean 52 ) .
	manualset3
171937	8	413322	7	NULL	NULL	0	NULL	follow-up	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Actuarial survivals at 8 years were 68 % , 44 % , and 15 % , respectively ( p less than .01 ) , with 1 to 165 months of follow-up ( mean 52 ) .
	manualset3
171938	9	413322	7	NULL	NULL	0	NULL	mean 52	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Actuarial survivals at 8 years were 68 % , 44 % , and 15 % , respectively ( p less than .01 ) , with 1 to 165 months of follow-up ( mean 52 ) .
	manualset3
171939	1	413323	7	NULL	NULL	0	NULL	suppression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , it is likely that suppression of TRPV6 by a hCa diet is required for its protective effects in the colon .
	manualset3
171940	2	413323	7	NULL	NULL	0	NULL	TRPV6	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , it is likely that suppression of TRPV6 by a hCa diet is required for its protective effects in the colon .
	manualset3
171941	3	413323	7	NULL	NULL	0	NULL	hCa diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , it is likely that suppression of TRPV6 by a hCa diet is required for its protective effects in the colon .
	manualset3
171942	4	413323	7	NULL	NULL	0	NULL	 protective effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , it is likely that suppression of TRPV6 by a hCa diet is required for its protective effects in the colon .
	manualset3
171943	5	413323	7	NULL	NULL	0	NULL	colon	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , it is likely that suppression of TRPV6 by a hCa diet is required for its protective effects in the colon .
	manualset3
171944	1	413324	7	NULL	NULL	0	NULL	techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , most techniques presented hitherto rely on single-plane imaging to visualize the catheter .
	manualset3
171945	2	413324	7	NULL	NULL	0	NULL	 single-plane imaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , most techniques presented hitherto rely on single-plane imaging to visualize the catheter .
	manualset3
171946	3	413324	7	NULL	NULL	0	NULL	catheter	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , most techniques presented hitherto rely on single-plane imaging to visualize the catheter .
	manualset3
171947	1	413325	7	NULL	NULL	0	NULL	environmental factors	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , other environmental factors such as infections or trauma might determine which patients would be at increased risk for IDRs .
	manualset3
171948	2	413325	7	NULL	NULL	0	NULL	 infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , other environmental factors such as infections or trauma might determine which patients would be at increased risk for IDRs .
	manualset3
171949	3	413325	7	NULL	NULL	0	NULL	 trauma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , other environmental factors such as infections or trauma might determine which patients would be at increased risk for IDRs .
	manualset3
171950	4	413325	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , other environmental factors such as infections or trauma might determine which patients would be at increased risk for IDRs .
	manualset3
171951	5	413325	7	NULL	NULL	0	NULL	 increased risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , other environmental factors such as infections or trauma might determine which patients would be at increased risk for IDRs .
	manualset3
171952	6	413325	7	NULL	NULL	0	NULL	IDRs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , other environmental factors such as infections or trauma might determine which patients would be at increased risk for IDRs .
	manualset3
171953	1	413326	7	NULL	NULL	0	NULL	 plamsinogen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , plamsinogen was tested as a possible preventive agent in RDS due to HMD .
	manualset3
171954	2	413326	7	NULL	NULL	0	NULL	preventive agent	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , plamsinogen was tested as a possible preventive agent in RDS due to HMD .
	manualset3
171955	3	413326	7	NULL	NULL	0	NULL	RDS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , plamsinogen was tested as a possible preventive agent in RDS due to HMD .
	manualset3
171956	4	413326	7	NULL	NULL	0	NULL	HMD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , plamsinogen was tested as a possible preventive agent in RDS due to HMD .
	manualset3
171957	1	413327	7	NULL	NULL	0	NULL	reactive screening tests	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , reactive screening tests must be validated by a confirmatory test in order to reduce the probability of false positive results to an acceptably low level , i.e. below 1 % .
	manualset3
171958	2	413327	7	NULL	NULL	0	NULL	confirmatory test 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , reactive screening tests must be validated by a confirmatory test in order to reduce the probability of false positive results to an acceptably low level , i.e. below 1 % .
	manualset3
171959	3	413327	7	NULL	NULL	0	NULL	probability	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , reactive screening tests must be validated by a confirmatory test in order to reduce the probability of false positive results to an acceptably low level , i.e. below 1 % .
	manualset3
171960	4	413327	7	NULL	NULL	0	NULL	false positive results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , reactive screening tests must be validated by a confirmatory test in order to reduce the probability of false positive results to an acceptably low level , i.e. below 1 % .
	manualset3
171961	5	413327	7	NULL	NULL	0	NULL	 low level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , reactive screening tests must be validated by a confirmatory test in order to reduce the probability of false positive results to an acceptably low level , i.e. below 1 % .
	manualset3
171962	6	413327	7	NULL	NULL	NULL	NULL	 below 1 % 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , reactive screening tests must be validated by a confirmatory test in order to reduce the probability of false positive results to an acceptably low level , i.e. below 1 % .
	manualset3
171963	1	413328	7	NULL	NULL	0	NULL	reduced production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , reduced production of adrenal hormones ( i.e. , cortisol , DHEAS ) at baseline in active and untreated patients with polymyalgia rheumatica was detected .
	manualset3
171964	2	413328	7	NULL	NULL	0	NULL	adrenal hormones	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , reduced production of adrenal hormones ( i.e. , cortisol , DHEAS ) at baseline in active and untreated patients with polymyalgia rheumatica was detected .
	manualset3
171965	3	413328	7	NULL	NULL	0	NULL	 cortisol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , reduced production of adrenal hormones ( i.e. , cortisol , DHEAS ) at baseline in active and untreated patients with polymyalgia rheumatica was detected .
	manualset3
171966	4	413328	7	NULL	NULL	0	NULL	DHEAS	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , reduced production of adrenal hormones ( i.e. , cortisol , DHEAS ) at baseline in active and untreated patients with polymyalgia rheumatica was detected .
	manualset3
171967	5	413328	7	NULL	NULL	0	NULL	baseline	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , reduced production of adrenal hormones ( i.e. , cortisol , DHEAS ) at baseline in active and untreated patients with polymyalgia rheumatica was detected .
	manualset3
171968	6	413328	7	NULL	NULL	0	NULL	active and untreated patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , reduced production of adrenal hormones ( i.e. , cortisol , DHEAS ) at baseline in active and untreated patients with polymyalgia rheumatica was detected .
	manualset3
171969	7	413328	7	NULL	NULL	0	NULL	polymyalgia rheumatica	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , reduced production of adrenal hormones ( i.e. , cortisol , DHEAS ) at baseline in active and untreated patients with polymyalgia rheumatica was detected .
	manualset3
171970	1	413329	7	NULL	NULL	0	NULL	reliable evaluation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , reliable evaluation of ( F ) ISH signals to screen for genomic changes was until now mainly restricted to isolated nuclei obtained from relatively thick tissue sections .
	manualset3
171971	2	413329	7	NULL	NULL	0	NULL	( F ) ISH signals	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , reliable evaluation of ( F ) ISH signals to screen for genomic changes was until now mainly restricted to isolated nuclei obtained from relatively thick tissue sections .
	manualset3
171972	3	413329	7	NULL	NULL	0	NULL	 genomic changes 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , reliable evaluation of ( F ) ISH signals to screen for genomic changes was until now mainly restricted to isolated nuclei obtained from relatively thick tissue sections .
	manualset3
171973	4	413329	7	NULL	NULL	0	NULL	isolated nuclei 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , reliable evaluation of ( F ) ISH signals to screen for genomic changes was until now mainly restricted to isolated nuclei obtained from relatively thick tissue sections .
	manualset3
171974	5	413329	7	NULL	NULL	0	NULL	thick tissue sections	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , reliable evaluation of ( F ) ISH signals to screen for genomic changes was until now mainly restricted to isolated nuclei obtained from relatively thick tissue sections .
	manualset3
171975	1	413330	7	NULL	NULL	0	NULL	schizophrenia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , schizophrenia , as we now know it , simply does not have an evolutionary history .
	manualset3
171976	2	413330	7	NULL	NULL	0	NULL	evolutionary history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , schizophrenia , as we now know it , simply does not have an evolutionary history .
	manualset3
171983	1	413331	7	NULL	NULL	0	NULL	spleen cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , spleen cells of the immunized animal are used to fuse with the respective species of myeloma cells to create in vitro immortalized antibodies secreting hybridomas .
	manualset3
171984	2	413331	7	NULL	NULL	0	NULL	 immunized animal	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , spleen cells of the immunized animal are used to fuse with the respective species of myeloma cells to create in vitro immortalized antibodies secreting hybridomas .
	manualset3
171985	3	413331	7	NULL	NULL	0	NULL	species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , spleen cells of the immunized animal are used to fuse with the respective species of myeloma cells to create in vitro immortalized antibodies secreting hybridomas .
	manualset3
171986	4	413331	7	NULL	NULL	0	NULL	myeloma cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , spleen cells of the immunized animal are used to fuse with the respective species of myeloma cells to create in vitro immortalized antibodies secreting hybridomas .
	manualset3
171987	5	413331	7	NULL	NULL	0	NULL	 in vitro immortalized antibodies secreting hybridomas	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , spleen cells of the immunized animal are used to fuse with the respective species of myeloma cells to create in vitro immortalized antibodies secreting hybridomas .
	manualset3
171988	1	413332	7	NULL	NULL	NULL	NULL	Actuarial 3 -year survival	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Actuarial 3 - and 5-year survival for benign disease was 95 % and 83 % and for malignant disease 52 % and 44 % , respectively ( P = 0.0048 ) .
	manualset3
171989	2	413332	7	NULL	NULL	NULL	NULL	Actuarial 5-year survival	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Actuarial 3 - and 5-year survival for benign disease was 95 % and 83 % and for malignant disease 52 % and 44 % , respectively ( P = 0.0048 ) .
	manualset3
171990	3	413332	7	NULL	NULL	NULL	NULL	benign disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Actuarial 3 - and 5-year survival for benign disease was 95 % and 83 % and for malignant disease 52 % and 44 % , respectively ( P = 0.0048 ) .
	manualset3
171991	4	413332	7	NULL	NULL	0	NULL	 95 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Actuarial 3 - and 5-year survival for benign disease was 95 % and 83 % and for malignant disease 52 % and 44 % , respectively ( P = 0.0048 ) .
	manualset3
171992	5	413332	7	NULL	NULL	0	NULL	 83 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Actuarial 3 - and 5-year survival for benign disease was 95 % and 83 % and for malignant disease 52 % and 44 % , respectively ( P = 0.0048 ) .
	manualset3
171993	6	413332	7	NULL	NULL	NULL	NULL	malignant disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Actuarial 3 - and 5-year survival for benign disease was 95 % and 83 % and for malignant disease 52 % and 44 % , respectively ( P = 0.0048 ) .
	manualset3
171994	7	413332	7	NULL	NULL	0	NULL	52 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Actuarial 3 - and 5-year survival for benign disease was 95 % and 83 % and for malignant disease 52 % and 44 % , respectively ( P = 0.0048 ) .
	manualset3
171995	8	413332	7	NULL	NULL	0	NULL	44 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Actuarial 3 - and 5-year survival for benign disease was 95 % and 83 % and for malignant disease 52 % and 44 % , respectively ( P = 0.0048 ) .
	manualset3
171996	9	413332	7	NULL	NULL	0	NULL	P = 0.0048	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Actuarial 3 - and 5-year survival for benign disease was 95 % and 83 % and for malignant disease 52 % and 44 % , respectively ( P = 0.0048 ) .
	manualset3
171997	1	413333	7	NULL	NULL	0	NULL	CCMM design	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the CCMM design that is proposed here is more suitable than the CMM for the construction of chiral metamaterials with a negative index .
	manualset3
171998	2	413333	7	NULL	NULL	0	NULL	CMM	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the CCMM design that is proposed here is more suitable than the CMM for the construction of chiral metamaterials with a negative index .
	manualset3
171999	3	413333	7	NULL	NULL	0	NULL	 construction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the CCMM design that is proposed here is more suitable than the CMM for the construction of chiral metamaterials with a negative index .
	manualset3
172000	4	413333	7	NULL	NULL	0	NULL	chiral metamaterials	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the CCMM design that is proposed here is more suitable than the CMM for the construction of chiral metamaterials with a negative index .
	manualset3
172001	5	413333	7	NULL	NULL	0	NULL	negative index	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the CCMM design that is proposed here is more suitable than the CMM for the construction of chiral metamaterials with a negative index .
	manualset3
172002	1	413334	7	NULL	NULL	0	NULL	S-layer-OM complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the S-layer-OM complex of T. thermophilus binds to the cell wall through the SLH motif of the S-layer protein via a strong interaction with a highly immunogenic pyruvylated component of the SCWP .
	manualset3
172003	2	413334	7	NULL	NULL	0	NULL	T. thermophilus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the S-layer-OM complex of T. thermophilus binds to the cell wall through the SLH motif of the S-layer protein via a strong interaction with a highly immunogenic pyruvylated component of the SCWP .
	manualset3
172004	3	413334	7	NULL	NULL	0	NULL	cell wall	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the S-layer-OM complex of T. thermophilus binds to the cell wall through the SLH motif of the S-layer protein via a strong interaction with a highly immunogenic pyruvylated component of the SCWP .
	manualset3
172005	4	413334	7	NULL	NULL	0	NULL	SLH motif	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the S-layer-OM complex of T. thermophilus binds to the cell wall through the SLH motif of the S-layer protein via a strong interaction with a highly immunogenic pyruvylated component of the SCWP .
	manualset3
172006	5	413334	7	NULL	NULL	0	NULL	S-layer protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the S-layer-OM complex of T. thermophilus binds to the cell wall through the SLH motif of the S-layer protein via a strong interaction with a highly immunogenic pyruvylated component of the SCWP .
	manualset3
172007	6	413334	7	NULL	NULL	0	NULL	strong interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the S-layer-OM complex of T. thermophilus binds to the cell wall through the SLH motif of the S-layer protein via a strong interaction with a highly immunogenic pyruvylated component of the SCWP .
	manualset3
172008	7	413334	7	NULL	NULL	NULL	NULL	immunogenic pyruvylated component 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , the S-layer-OM complex of T. thermophilus binds to the cell wall through the SLH motif of the S-layer protein via a strong interaction with a highly immunogenic pyruvylated component of the SCWP .
	manualset3
172009	8	413334	7	NULL	NULL	0	NULL	SCWP	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the S-layer-OM complex of T. thermophilus binds to the cell wall through the SLH motif of the S-layer protein via a strong interaction with a highly immunogenic pyruvylated component of the SCWP .
	manualset3
172010	1	413335	7	NULL	NULL	0	NULL	aim 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the aim of the present study was to investigate the effects of macrophage migration inhibitory factor on spinal cord neuron survival and viability .
	manualset3
172011	2	413335	7	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the aim of the present study was to investigate the effects of macrophage migration inhibitory factor on spinal cord neuron survival and viability .
	manualset3
172012	3	413335	7	NULL	NULL	0	NULL	 effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the aim of the present study was to investigate the effects of macrophage migration inhibitory factor on spinal cord neuron survival and viability .
	manualset3
172013	4	413335	7	NULL	NULL	0	NULL	macrophage migration inhibitory factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the aim of the present study was to investigate the effects of macrophage migration inhibitory factor on spinal cord neuron survival and viability .
	manualset3
172014	5	413335	7	NULL	NULL	0	NULL	spinal cord neuron survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the aim of the present study was to investigate the effects of macrophage migration inhibitory factor on spinal cord neuron survival and viability .
	manualset3
172015	6	413335	7	NULL	NULL	0	NULL	viability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the aim of the present study was to investigate the effects of macrophage migration inhibitory factor on spinal cord neuron survival and viability .
	manualset3
172020	1	413336	7	NULL	NULL	0	NULL	aim	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the aim of the study was to characterize the phosphorylation of recombinant human Gab-1 ( hGab-1 ) protein by EGFR in vitro .
	manualset3
172021	2	413336	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the aim of the study was to characterize the phosphorylation of recombinant human Gab-1 ( hGab-1 ) protein by EGFR in vitro .
	manualset3
172022	3	413336	7	NULL	NULL	0	NULL	phosphorylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the aim of the study was to characterize the phosphorylation of recombinant human Gab-1 ( hGab-1 ) protein by EGFR in vitro .
	manualset3
172023	4	413336	7	NULL	NULL	0	NULL	recombinant human Gab-1 ( hGab-1 ) protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the aim of the study was to characterize the phosphorylation of recombinant human Gab-1 ( hGab-1 ) protein by EGFR in vitro .
	manualset3
172024	5	413336	7	NULL	NULL	0	NULL	EGFR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the aim of the study was to characterize the phosphorylation of recombinant human Gab-1 ( hGab-1 ) protein by EGFR in vitro .
	manualset3
172025	1	413337	7	NULL	NULL	0	NULL	 antibody response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the antibody response to influenza vaccination was assessed in a postmenopausal mouse model .
	manualset3
172026	2	413337	7	NULL	NULL	0	NULL	influenza vaccination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the antibody response to influenza vaccination was assessed in a postmenopausal mouse model .
	manualset3
172027	3	413337	7	NULL	NULL	NULL	NULL	postmenopausal mouse model	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , the antibody response to influenza vaccination was assessed in a postmenopausal mouse model .
	manualset3
172028	1	413338	7	NULL	NULL	0	NULL	 catalytic mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the catalytic mechanisms of type-I MetAPs may differ somewhat from type-II enzymes when a dinuclear metalloactive site is present .
	manualset3
172029	2	413338	7	NULL	NULL	NULL	NULL	type-I MetAPs	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , the catalytic mechanisms of type-I MetAPs may differ somewhat from type-II enzymes when a dinuclear metalloactive site is present .
	manualset3
172030	3	413338	7	NULL	NULL	0	NULL	type-II enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the catalytic mechanisms of type-I MetAPs may differ somewhat from type-II enzymes when a dinuclear metalloactive site is present .
	manualset3
172031	4	413338	7	NULL	NULL	0	NULL	dinuclear metalloactive site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the catalytic mechanisms of type-I MetAPs may differ somewhat from type-II enzymes when a dinuclear metalloactive site is present .
	manualset3
172032	1	413339	7	NULL	NULL	0	NULL	Acute toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute , subacute and chronic toxicity of fosfosal .
	manualset3
172033	2	413339	7	NULL	NULL	0	NULL	subacute toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute , subacute and chronic toxicity of fosfosal .
	manualset3
172034	3	413339	7	NULL	NULL	0	NULL	chronic toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute , subacute and chronic toxicity of fosfosal .
	manualset3
172035	4	413339	7	NULL	NULL	0	NULL	fosfosal	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute , subacute and chronic toxicity of fosfosal .
	manualset3
172036	1	413340	7	NULL	NULL	0	NULL	covalent C3b-binding site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the covalent C3b-binding site on C4b is located within a 74-residue region of the primary structure .
	manualset3
172037	2	413340	7	NULL	NULL	0	NULL	 C4b	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the covalent C3b-binding site on C4b is located within a 74-residue region of the primary structure .
	manualset3
172038	3	413340	7	NULL	NULL	0	NULL	74-residue region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the covalent C3b-binding site on C4b is located within a 74-residue region of the primary structure .
	manualset3
172039	4	413340	7	NULL	NULL	0	NULL	primary structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the covalent C3b-binding site on C4b is located within a 74-residue region of the primary structure .
	manualset3
172040	1	413341	7	NULL	NULL	0	NULL	developmental regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the developmental regulation of PP2A activity and protein during kidney development and its mapping to the nephrogenic cortex , developing glomeruli , and tubules suggests a role for PP2A in the regulation of nephron growth and differentiation .
	manualset3
172041	2	413341	7	NULL	NULL	0	NULL	PP2A activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the developmental regulation of PP2A activity and protein during kidney development and its mapping to the nephrogenic cortex , developing glomeruli , and tubules suggests a role for PP2A in the regulation of nephron growth and differentiation .
	manualset3
172042	3	413341	7	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the developmental regulation of PP2A activity and protein during kidney development and its mapping to the nephrogenic cortex , developing glomeruli , and tubules suggests a role for PP2A in the regulation of nephron growth and differentiation .
	manualset3
172043	4	413341	7	NULL	NULL	0	NULL	kidney development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the developmental regulation of PP2A activity and protein during kidney development and its mapping to the nephrogenic cortex , developing glomeruli , and tubules suggests a role for PP2A in the regulation of nephron growth and differentiation .
	manualset3
172044	5	413341	7	NULL	NULL	0	NULL	mapping	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the developmental regulation of PP2A activity and protein during kidney development and its mapping to the nephrogenic cortex , developing glomeruli , and tubules suggests a role for PP2A in the regulation of nephron growth and differentiation .
	manualset3
172045	6	413341	7	NULL	NULL	0	NULL	nephrogenic cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the developmental regulation of PP2A activity and protein during kidney development and its mapping to the nephrogenic cortex , developing glomeruli , and tubules suggests a role for PP2A in the regulation of nephron growth and differentiation .
	manualset3
172046	7	413341	7	NULL	NULL	0	NULL	developing glomeruli	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the developmental regulation of PP2A activity and protein during kidney development and its mapping to the nephrogenic cortex , developing glomeruli , and tubules suggests a role for PP2A in the regulation of nephron growth and differentiation .
	manualset3
172047	8	413341	7	NULL	NULL	0	NULL	 tubules	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the developmental regulation of PP2A activity and protein during kidney development and its mapping to the nephrogenic cortex , developing glomeruli , and tubules suggests a role for PP2A in the regulation of nephron growth and differentiation .
	manualset3
172048	9	413341	7	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the developmental regulation of PP2A activity and protein during kidney development and its mapping to the nephrogenic cortex , developing glomeruli , and tubules suggests a role for PP2A in the regulation of nephron growth and differentiation .
	manualset3
172049	10	413341	7	NULL	NULL	0	NULL	PP2A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the developmental regulation of PP2A activity and protein during kidney development and its mapping to the nephrogenic cortex , developing glomeruli , and tubules suggests a role for PP2A in the regulation of nephron growth and differentiation .
	manualset3
172050	11	413341	7	NULL	NULL	0	NULL	regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the developmental regulation of PP2A activity and protein during kidney development and its mapping to the nephrogenic cortex , developing glomeruli , and tubules suggests a role for PP2A in the regulation of nephron growth and differentiation .
	manualset3
172051	12	413341	7	NULL	NULL	0	NULL	nephron growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the developmental regulation of PP2A activity and protein during kidney development and its mapping to the nephrogenic cortex , developing glomeruli , and tubules suggests a role for PP2A in the regulation of nephron growth and differentiation .
	manualset3
172052	13	413341	7	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the developmental regulation of PP2A activity and protein during kidney development and its mapping to the nephrogenic cortex , developing glomeruli , and tubules suggests a role for PP2A in the regulation of nephron growth and differentiation .
	manualset3
172053	1	413342	7	NULL	NULL	0	NULL	 distensibility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the distensibility or compliance at the long prosthesis seems to be very important in cases with long grafts of the aorta .
	manualset3
172054	2	413342	7	NULL	NULL	0	NULL	compliance at the long prosthesis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the distensibility or compliance at the long prosthesis seems to be very important in cases with long grafts of the aorta .
	manualset3
172055	3	413342	7	NULL	NULL	0	NULL	cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the distensibility or compliance at the long prosthesis seems to be very important in cases with long grafts of the aorta .
	manualset3
172056	4	413342	7	NULL	NULL	NULL	NULL	long grafts	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , the distensibility or compliance at the long prosthesis seems to be very important in cases with long grafts of the aorta .
	manualset3
173618	5	413342	7	NULL	NULL	0	NULL	aorta	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the distensibility or compliance at the long prosthesis seems to be very important in cases with long grafts of the aorta .
	manualset3
172057	1	413343	7	NULL	NULL	NULL	NULL	 effect	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , the effect of replacement of FSH , GH , diethylstilbestrol ( DES ) , or combinations thereof was evaluated .
	manualset3
172058	2	413343	7	NULL	NULL	NULL	NULL	FSH	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , the effect of replacement of FSH , GH , diethylstilbestrol ( DES ) , or combinations thereof was evaluated .
	manualset3
172059	3	413343	7	NULL	NULL	NULL	NULL	 GH	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , the effect of replacement of FSH , GH , diethylstilbestrol ( DES ) , or combinations thereof was evaluated .
	manualset3
172060	4	413343	7	NULL	NULL	NULL	NULL	diethylstilbestrol ( DES )	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , the effect of replacement of FSH , GH , diethylstilbestrol ( DES ) , or combinations thereof was evaluated .
	manualset3
172061	5	413343	7	NULL	NULL	NULL	NULL	 combinations	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , the effect of replacement of FSH , GH , diethylstilbestrol ( DES ) , or combinations thereof was evaluated .
	manualset3
172062	6	413343	7	NULL	NULL	0	NULL	replacement	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the effect of replacement of FSH , GH , diethylstilbestrol ( DES ) , or combinations thereof was evaluated .
	manualset3
172063	1	413344	7	NULL	NULL	0	NULL	incorporation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the incorporation of LEO into gelatin film could enhance the antimicrobial and antioxidative properties of the film , thereby maintaining the qualities and extending the shelf-life of the sea bass slices stored at refrigerated temperature .
	manualset3
172064	2	413344	7	NULL	NULL	0	NULL	 LEO	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the incorporation of LEO into gelatin film could enhance the antimicrobial and antioxidative properties of the film , thereby maintaining the qualities and extending the shelf-life of the sea bass slices stored at refrigerated temperature .
	manualset3
172065	3	413344	7	NULL	NULL	0	NULL	gelatin film	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the incorporation of LEO into gelatin film could enhance the antimicrobial and antioxidative properties of the film , thereby maintaining the qualities and extending the shelf-life of the sea bass slices stored at refrigerated temperature .
	manualset3
172066	4	413344	7	NULL	NULL	0	NULL	 antimicrobial properties	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the incorporation of LEO into gelatin film could enhance the antimicrobial and antioxidative properties of the film , thereby maintaining the qualities and extending the shelf-life of the sea bass slices stored at refrigerated temperature .
	manualset3
172067	5	413344	7	NULL	NULL	0	NULL	antioxidative properties	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the incorporation of LEO into gelatin film could enhance the antimicrobial and antioxidative properties of the film , thereby maintaining the qualities and extending the shelf-life of the sea bass slices stored at refrigerated temperature .
	manualset3
172068	6	413344	7	NULL	NULL	0	NULL	film	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the incorporation of LEO into gelatin film could enhance the antimicrobial and antioxidative properties of the film , thereby maintaining the qualities and extending the shelf-life of the sea bass slices stored at refrigerated temperature .
	manualset3
172069	7	413344	7	NULL	NULL	0	NULL	shelf-life	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the incorporation of LEO into gelatin film could enhance the antimicrobial and antioxidative properties of the film , thereby maintaining the qualities and extending the shelf-life of the sea bass slices stored at refrigerated temperature .
	manualset3
172070	8	413344	7	NULL	NULL	0	NULL	sea bass slices	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the incorporation of LEO into gelatin film could enhance the antimicrobial and antioxidative properties of the film , thereby maintaining the qualities and extending the shelf-life of the sea bass slices stored at refrigerated temperature .
	manualset3
172071	9	413344	7	NULL	NULL	0	NULL	refrigerated temperature	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the incorporation of LEO into gelatin film could enhance the antimicrobial and antioxidative properties of the film , thereby maintaining the qualities and extending the shelf-life of the sea bass slices stored at refrigerated temperature .
	manualset3
173619	10	413344	7	NULL	NULL	0	NULL	qualities	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the incorporation of LEO into gelatin film could enhance the antimicrobial and antioxidative properties of the film , thereby maintaining the qualities and extending the shelf-life of the sea bass slices stored at refrigerated temperature .
	manualset3
172072	1	413345	7	NULL	NULL	0	NULL	knowledge	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the knowledge of the enantiomeric composition of alpha-terpineol and linalool might be useful for thermal treatment control purposes .
	manualset3
172073	2	413345	7	NULL	NULL	0	NULL	 enantiomeric composition 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the knowledge of the enantiomeric composition of alpha-terpineol and linalool might be useful for thermal treatment control purposes .
	manualset3
172074	3	413345	7	NULL	NULL	0	NULL	 alpha-terpineol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the knowledge of the enantiomeric composition of alpha-terpineol and linalool might be useful for thermal treatment control purposes .
	manualset3
172075	4	413345	7	NULL	NULL	0	NULL	 linalool 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the knowledge of the enantiomeric composition of alpha-terpineol and linalool might be useful for thermal treatment control purposes .
	manualset3
172076	5	413345	7	NULL	NULL	0	NULL	thermal treatment control purposes	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the knowledge of the enantiomeric composition of alpha-terpineol and linalool might be useful for thermal treatment control purposes .
	manualset3
172077	1	413346	7	NULL	NULL	0	NULL	method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the most efficient method for Hb purification appears to be clarification with a 50 nm tangential flow filter , followed by purification with IMAC , and sample concentration/polishing on a 10-50 kDa tangential flow filter .
	manualset3
172078	2	413346	7	NULL	NULL	0	NULL	Hb purification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the most efficient method for Hb purification appears to be clarification with a 50 nm tangential flow filter , followed by purification with IMAC , and sample concentration/polishing on a 10-50 kDa tangential flow filter .
	manualset3
172079	3	413346	7	NULL	NULL	0	NULL	50 nm tangential flow filter	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the most efficient method for Hb purification appears to be clarification with a 50 nm tangential flow filter , followed by purification with IMAC , and sample concentration/polishing on a 10-50 kDa tangential flow filter .
	manualset3
172080	4	413346	7	NULL	NULL	0	NULL	purification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the most efficient method for Hb purification appears to be clarification with a 50 nm tangential flow filter , followed by purification with IMAC , and sample concentration/polishing on a 10-50 kDa tangential flow filter .
	manualset3
172081	5	413346	7	NULL	NULL	0	NULL	IMAC	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the most efficient method for Hb purification appears to be clarification with a 50 nm tangential flow filter , followed by purification with IMAC , and sample concentration/polishing on a 10-50 kDa tangential flow filter .
	manualset3
172082	6	413346	7	NULL	NULL	0	NULL	sample concentration/polishing 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the most efficient method for Hb purification appears to be clarification with a 50 nm tangential flow filter , followed by purification with IMAC , and sample concentration/polishing on a 10-50 kDa tangential flow filter .
	manualset3
172083	7	413346	7	NULL	NULL	NULL	NULL	10-50 kDa	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , the most efficient method for Hb purification appears to be clarification with a 50 nm tangential flow filter , followed by purification with IMAC , and sample concentration/polishing on a 10-50 kDa tangential flow filter .
	manualset3
173620	8	413346	7	NULL	NULL	0	NULL	clarification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the most efficient method for Hb purification appears to be clarification with a 50 nm tangential flow filter , followed by purification with IMAC , and sample concentration/polishing on a 10-50 kDa tangential flow filter .
	manualset3
173656	9	413346	7	NULL	NULL	0	NULL	 tangential flow filter	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the most efficient method for Hb purification appears to be clarification with a 50 nm tangential flow filter , followed by purification with IMAC , and sample concentration/polishing on a 10-50 kDa tangential flow filter .
	manualset3
172084	1	413347	7	NULL	NULL	0	NULL	Acute ablation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute ablation of AgRP neurons in adult mice by the action of diphtheria toxin ( DT ) results in precipitous reduction of food intake , and eventually leads to starvation within 6days of DT treatment .
	manualset3
172085	2	413347	7	NULL	NULL	NULL	NULL	AgRP neurons	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Acute ablation of AgRP neurons in adult mice by the action of diphtheria toxin ( DT ) results in precipitous reduction of food intake , and eventually leads to starvation within 6days of DT treatment .
	manualset3
172086	3	413347	7	NULL	NULL	0	NULL	adult mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute ablation of AgRP neurons in adult mice by the action of diphtheria toxin ( DT ) results in precipitous reduction of food intake , and eventually leads to starvation within 6days of DT treatment .
	manualset3
172087	4	413347	7	NULL	NULL	NULL	NULL	action 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Acute ablation of AgRP neurons in adult mice by the action of diphtheria toxin ( DT ) results in precipitous reduction of food intake , and eventually leads to starvation within 6days of DT treatment .
	manualset3
172088	5	413347	7	NULL	NULL	0	NULL	diphtheria toxin ( DT )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute ablation of AgRP neurons in adult mice by the action of diphtheria toxin ( DT ) results in precipitous reduction of food intake , and eventually leads to starvation within 6days of DT treatment .
	manualset3
172089	6	413347	7	NULL	NULL	NULL	NULL	precipitous reduction	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Acute ablation of AgRP neurons in adult mice by the action of diphtheria toxin ( DT ) results in precipitous reduction of food intake , and eventually leads to starvation within 6days of DT treatment .
	manualset3
172090	7	413347	7	NULL	NULL	0	NULL	food intake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute ablation of AgRP neurons in adult mice by the action of diphtheria toxin ( DT ) results in precipitous reduction of food intake , and eventually leads to starvation within 6days of DT treatment .
	manualset3
172091	8	413347	7	NULL	NULL	0	NULL	starvation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute ablation of AgRP neurons in adult mice by the action of diphtheria toxin ( DT ) results in precipitous reduction of food intake , and eventually leads to starvation within 6days of DT treatment .
	manualset3
172092	9	413347	7	NULL	NULL	0	NULL	 6days 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute ablation of AgRP neurons in adult mice by the action of diphtheria toxin ( DT ) results in precipitous reduction of food intake , and eventually leads to starvation within 6days of DT treatment .
	manualset3
172093	10	413347	7	NULL	NULL	0	NULL	DT treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute ablation of AgRP neurons in adult mice by the action of diphtheria toxin ( DT ) results in precipitous reduction of food intake , and eventually leads to starvation within 6days of DT treatment .
	manualset3
172094	1	413348	7	NULL	NULL	0	NULL	objective	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the objective of the current study was to develop such a phenotypic cell-based assay for measuring the forward mutation rate of HIV-1 .
	manualset3
172095	2	413348	7	NULL	NULL	0	NULL	current study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the objective of the current study was to develop such a phenotypic cell-based assay for measuring the forward mutation rate of HIV-1 .
	manualset3
172096	3	413348	7	NULL	NULL	0	NULL	phenotypic cell-based assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the objective of the current study was to develop such a phenotypic cell-based assay for measuring the forward mutation rate of HIV-1 .
	manualset3
172097	4	413348	7	NULL	NULL	0	NULL	forward mutation rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the objective of the current study was to develop such a phenotypic cell-based assay for measuring the forward mutation rate of HIV-1 .
	manualset3
172098	5	413348	7	NULL	NULL	0	NULL	HIV-1	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the objective of the current study was to develop such a phenotypic cell-based assay for measuring the forward mutation rate of HIV-1 .
	manualset3
172099	1	413349	7	NULL	NULL	0	NULL	 involvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the possible involvement of gonadal steroids in the regulation of brain AR1 levels was investigated in the present study .
	manualset3
172100	2	413349	7	NULL	NULL	0	NULL	gonadal steroids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the possible involvement of gonadal steroids in the regulation of brain AR1 levels was investigated in the present study .
	manualset3
172101	3	413349	7	NULL	NULL	NULL	NULL	regulation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , the possible involvement of gonadal steroids in the regulation of brain AR1 levels was investigated in the present study .
	manualset3
172102	4	413349	7	NULL	NULL	0	NULL	brain AR1 levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the possible involvement of gonadal steroids in the regulation of brain AR1 levels was investigated in the present study .
	manualset3
172103	5	413349	7	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the possible involvement of gonadal steroids in the regulation of brain AR1 levels was investigated in the present study .
	manualset3
172104	1	413350	7	NULL	NULL	0	NULL	 proliferation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the proliferation and differentiation capacity in primary cultures of adipose tissue-derived stromal cells were compared between the 2 depots in a group of 29 obese individuals , of which 21 were women .
	manualset3
172105	2	413350	7	NULL	NULL	0	NULL	differentiation capacity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the proliferation and differentiation capacity in primary cultures of adipose tissue-derived stromal cells were compared between the 2 depots in a group of 29 obese individuals , of which 21 were women .
	manualset3
172106	3	413350	7	NULL	NULL	0	NULL	primary cultures	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the proliferation and differentiation capacity in primary cultures of adipose tissue-derived stromal cells were compared between the 2 depots in a group of 29 obese individuals , of which 21 were women .
	manualset3
172107	4	413350	7	NULL	NULL	0	NULL	adipose tissue-derived stromal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the proliferation and differentiation capacity in primary cultures of adipose tissue-derived stromal cells were compared between the 2 depots in a group of 29 obese individuals , of which 21 were women .
	manualset3
172108	5	413350	7	NULL	NULL	0	NULL	2 depots	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the proliferation and differentiation capacity in primary cultures of adipose tissue-derived stromal cells were compared between the 2 depots in a group of 29 obese individuals , of which 21 were women .
	manualset3
172109	6	413350	7	NULL	NULL	0	NULL	group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the proliferation and differentiation capacity in primary cultures of adipose tissue-derived stromal cells were compared between the 2 depots in a group of 29 obese individuals , of which 21 were women .
	manualset3
172110	7	413350	7	NULL	NULL	0	NULL	29 obese individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the proliferation and differentiation capacity in primary cultures of adipose tissue-derived stromal cells were compared between the 2 depots in a group of 29 obese individuals , of which 21 were women .
	manualset3
172111	8	413350	7	NULL	NULL	0	NULL	21	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the proliferation and differentiation capacity in primary cultures of adipose tissue-derived stromal cells were compared between the 2 depots in a group of 29 obese individuals , of which 21 were women .
	manualset3
172112	9	413350	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the proliferation and differentiation capacity in primary cultures of adipose tissue-derived stromal cells were compared between the 2 depots in a group of 29 obese individuals , of which 21 were women .
	manualset3
172113	1	413351	7	NULL	NULL	0	NULL	requirement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the requirement for ancillary factors appears to be , in certain instances , dictated by the intrinsic properties of individual OM proteins , conceivably reflecting their propensities to misfold during periplasmic transit .
	manualset3
172114	2	413351	7	NULL	NULL	0	NULL	 ancillary factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the requirement for ancillary factors appears to be , in certain instances , dictated by the intrinsic properties of individual OM proteins , conceivably reflecting their propensities to misfold during periplasmic transit .
	manualset3
172115	3	413351	7	NULL	NULL	0	NULL	intrinsic properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the requirement for ancillary factors appears to be , in certain instances , dictated by the intrinsic properties of individual OM proteins , conceivably reflecting their propensities to misfold during periplasmic transit .
	manualset3
172116	4	413351	7	NULL	NULL	0	NULL	individual OM proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the requirement for ancillary factors appears to be , in certain instances , dictated by the intrinsic properties of individual OM proteins , conceivably reflecting their propensities to misfold during periplasmic transit .
	manualset3
172117	5	413351	7	NULL	NULL	0	NULL	propensities	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the requirement for ancillary factors appears to be , in certain instances , dictated by the intrinsic properties of individual OM proteins , conceivably reflecting their propensities to misfold during periplasmic transit .
	manualset3
172118	6	413351	7	NULL	NULL	0	NULL	periplasmic transit 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the requirement for ancillary factors appears to be , in certain instances , dictated by the intrinsic properties of individual OM proteins , conceivably reflecting their propensities to misfold during periplasmic transit .
	manualset3
172119	1	413352	7	NULL	NULL	0	NULL	resistance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the resistance to enzyme digestion of a specific processed starch is the result of a competition between the kinetics of enzyme hydrolysis and the kinetics of amylose retrogradation .
	manualset3
172120	2	413352	7	NULL	NULL	0	NULL	 enzyme digestion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the resistance to enzyme digestion of a specific processed starch is the result of a competition between the kinetics of enzyme hydrolysis and the kinetics of amylose retrogradation .
	manualset3
172121	3	413352	7	NULL	NULL	0	NULL	specific processed starch	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the resistance to enzyme digestion of a specific processed starch is the result of a competition between the kinetics of enzyme hydrolysis and the kinetics of amylose retrogradation .
	manualset3
172122	4	413352	7	NULL	NULL	0	NULL	 result	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the resistance to enzyme digestion of a specific processed starch is the result of a competition between the kinetics of enzyme hydrolysis and the kinetics of amylose retrogradation .
	manualset3
172123	5	413352	7	NULL	NULL	0	NULL	 competition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the resistance to enzyme digestion of a specific processed starch is the result of a competition between the kinetics of enzyme hydrolysis and the kinetics of amylose retrogradation .
	manualset3
172124	6	413352	7	NULL	NULL	NULL	NULL	 kinetics	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , the resistance to enzyme digestion of a specific processed starch is the result of a competition between the kinetics of enzyme hydrolysis and the kinetics of amylose retrogradation .
	manualset3
172125	7	413352	7	NULL	NULL	0	NULL	enzyme hydrolysis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the resistance to enzyme digestion of a specific processed starch is the result of a competition between the kinetics of enzyme hydrolysis and the kinetics of amylose retrogradation .
	manualset3
172126	8	413352	7	NULL	NULL	0	NULL	kinetics	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the resistance to enzyme digestion of a specific processed starch is the result of a competition between the kinetics of enzyme hydrolysis and the kinetics of amylose retrogradation .
	manualset3
172127	9	413352	7	NULL	NULL	0	NULL	amylose retrogradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the resistance to enzyme digestion of a specific processed starch is the result of a competition between the kinetics of enzyme hydrolysis and the kinetics of amylose retrogradation .
	manualset3
172128	1	413353	7	NULL	NULL	0	NULL	 suppression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the suppression of the negative wave by histamine and noradrenaline was mediated by the H1-receptor and alpha 1-receptor , respectively .
	manualset3
172129	2	413353	7	NULL	NULL	0	NULL	negative wave	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the suppression of the negative wave by histamine and noradrenaline was mediated by the H1-receptor and alpha 1-receptor , respectively .
	manualset3
172130	3	413353	7	NULL	NULL	0	NULL	histamine	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the suppression of the negative wave by histamine and noradrenaline was mediated by the H1-receptor and alpha 1-receptor , respectively .
	manualset3
172131	4	413353	7	NULL	NULL	0	NULL	noradrenaline	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the suppression of the negative wave by histamine and noradrenaline was mediated by the H1-receptor and alpha 1-receptor , respectively .
	manualset3
172132	5	413353	7	NULL	NULL	0	NULL	H1-receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the suppression of the negative wave by histamine and noradrenaline was mediated by the H1-receptor and alpha 1-receptor , respectively .
	manualset3
172133	6	413353	7	NULL	NULL	0	NULL	 alpha 1-receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the suppression of the negative wave by histamine and noradrenaline was mediated by the H1-receptor and alpha 1-receptor , respectively .
	manualset3
172134	1	413354	7	NULL	NULL	0	NULL	therapeutic strategies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , there is need for new therapeutic strategies not only to obtain higher treatment efficacy , but also for the reduction of toxicity and adverse effects .
	manualset3
172135	2	413354	7	NULL	NULL	0	NULL	treatment efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , there is need for new therapeutic strategies not only to obtain higher treatment efficacy , but also for the reduction of toxicity and adverse effects .
	manualset3
172136	3	413354	7	NULL	NULL	0	NULL	 reduction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , there is need for new therapeutic strategies not only to obtain higher treatment efficacy , but also for the reduction of toxicity and adverse effects .
	manualset3
172137	4	413354	7	NULL	NULL	0	NULL	toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , there is need for new therapeutic strategies not only to obtain higher treatment efficacy , but also for the reduction of toxicity and adverse effects .
	manualset3
172138	5	413354	7	NULL	NULL	0	NULL	adverse effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , there is need for new therapeutic strategies not only to obtain higher treatment efficacy , but also for the reduction of toxicity and adverse effects .
	manualset3
172139	1	413355	7	NULL	NULL	0	NULL	Acute aortic valve thrombosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute aortic valve thrombosis secondary to recombinant factor VIIa .
	manualset3
172140	2	413355	7	NULL	NULL	0	NULL	recombinant factor VIIa	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute aortic valve thrombosis secondary to recombinant factor VIIa .
	manualset3
172141	1	413356	7	NULL	NULL	0	NULL	alteration	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , there is no alteration of the quality of the platelets as evaluated with monoclonal antibodies ( MoAbs ) anti-CD 62 , 63 , 36 and 51 , no extra hemorrhagic risk for the donors and citrate reactions and microaggregate formation are totally eliminated .
	manualset3
172142	2	413356	7	NULL	NULL	0	NULL	 quality	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , there is no alteration of the quality of the platelets as evaluated with monoclonal antibodies ( MoAbs ) anti-CD 62 , 63 , 36 and 51 , no extra hemorrhagic risk for the donors and citrate reactions and microaggregate formation are totally eliminated .
	manualset3
172143	3	413356	7	NULL	NULL	0	NULL	platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , there is no alteration of the quality of the platelets as evaluated with monoclonal antibodies ( MoAbs ) anti-CD 62 , 63 , 36 and 51 , no extra hemorrhagic risk for the donors and citrate reactions and microaggregate formation are totally eliminated .
	manualset3
172144	4	413356	7	NULL	NULL	0	NULL	monoclonal antibodies ( MoAbs )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , there is no alteration of the quality of the platelets as evaluated with monoclonal antibodies ( MoAbs ) anti-CD 62 , 63 , 36 and 51 , no extra hemorrhagic risk for the donors and citrate reactions and microaggregate formation are totally eliminated .
	manualset3
172145	5	413356	7	NULL	NULL	0	NULL	 anti-CD 62	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , there is no alteration of the quality of the platelets as evaluated with monoclonal antibodies ( MoAbs ) anti-CD 62 , 63 , 36 and 51 , no extra hemorrhagic risk for the donors and citrate reactions and microaggregate formation are totally eliminated .
	manualset3
172146	6	413356	7	NULL	NULL	NULL	NULL	anti-CD 63	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , there is no alteration of the quality of the platelets as evaluated with monoclonal antibodies ( MoAbs ) anti-CD 62 , 63 , 36 and 51 , no extra hemorrhagic risk for the donors and citrate reactions and microaggregate formation are totally eliminated .
	manualset3
172147	7	413356	7	NULL	NULL	NULL	NULL	anti-CD 36	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , there is no alteration of the quality of the platelets as evaluated with monoclonal antibodies ( MoAbs ) anti-CD 62 , 63 , 36 and 51 , no extra hemorrhagic risk for the donors and citrate reactions and microaggregate formation are totally eliminated .
	manualset3
172148	8	413356	7	NULL	NULL	NULL	NULL	anti-CD 51	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , there is no alteration of the quality of the platelets as evaluated with monoclonal antibodies ( MoAbs ) anti-CD 62 , 63 , 36 and 51 , no extra hemorrhagic risk for the donors and citrate reactions and microaggregate formation are totally eliminated .
	manualset3
172149	9	413356	7	NULL	NULL	0	NULL	hemorrhagic risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , there is no alteration of the quality of the platelets as evaluated with monoclonal antibodies ( MoAbs ) anti-CD 62 , 63 , 36 and 51 , no extra hemorrhagic risk for the donors and citrate reactions and microaggregate formation are totally eliminated .
	manualset3
172150	10	413356	7	NULL	NULL	0	NULL	donors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , there is no alteration of the quality of the platelets as evaluated with monoclonal antibodies ( MoAbs ) anti-CD 62 , 63 , 36 and 51 , no extra hemorrhagic risk for the donors and citrate reactions and microaggregate formation are totally eliminated .
	manualset3
172151	11	413356	7	NULL	NULL	NULL	NULL	citrate reactions	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , there is no alteration of the quality of the platelets as evaluated with monoclonal antibodies ( MoAbs ) anti-CD 62 , 63 , 36 and 51 , no extra hemorrhagic risk for the donors and citrate reactions and microaggregate formation are totally eliminated .
	manualset3
172152	12	413356	7	NULL	NULL	NULL	NULL	microaggregate formation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , there is no alteration of the quality of the platelets as evaluated with monoclonal antibodies ( MoAbs ) anti-CD 62 , 63 , 36 and 51 , no extra hemorrhagic risk for the donors and citrate reactions and microaggregate formation are totally eliminated .
	manualset3
172153	1	413357	7	NULL	NULL	0	NULL	apparatus	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , this apparatus seems to be highly useful in the diagnosis of both ossicular chain disorders and eardrum perforations .
	manualset3
172154	2	413357	7	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , this apparatus seems to be highly useful in the diagnosis of both ossicular chain disorders and eardrum perforations .
	manualset3
172155	3	413357	7	NULL	NULL	0	NULL	ossicular chain disorders 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , this apparatus seems to be highly useful in the diagnosis of both ossicular chain disorders and eardrum perforations .
	manualset3
172156	4	413357	7	NULL	NULL	NULL	NULL	eardrum perforations	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , this apparatus seems to be highly useful in the diagnosis of both ossicular chain disorders and eardrum perforations .
	manualset3
172157	1	413358	7	NULL	NULL	NULL	NULL	approach	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , this approach suggests that PT-KP prodrug has a good colon targeting property .
	manualset3
172158	2	413358	7	NULL	NULL	0	NULL	PT-KP prodrug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , this approach suggests that PT-KP prodrug has a good colon targeting property .
	manualset3
172159	3	413358	7	NULL	NULL	0	NULL	good colon targeting property	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , this approach suggests that PT-KP prodrug has a good colon targeting property .
	manualset3
172160	1	413359	7	NULL	NULL	0	NULL	current study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , this current study is aimed to look for an alternative treatment by using Herniaria hirsuta on nephrolithiasic rats as a preventive agent against the development of kidney stones .
	manualset3
172161	2	413359	7	NULL	NULL	0	NULL	alternative treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , this current study is aimed to look for an alternative treatment by using Herniaria hirsuta on nephrolithiasic rats as a preventive agent against the development of kidney stones .
	manualset3
172162	3	413359	7	NULL	NULL	0	NULL	Herniaria hirsuta	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , this current study is aimed to look for an alternative treatment by using Herniaria hirsuta on nephrolithiasic rats as a preventive agent against the development of kidney stones .
	manualset3
172163	4	413359	7	NULL	NULL	0	NULL	nephrolithiasic rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , this current study is aimed to look for an alternative treatment by using Herniaria hirsuta on nephrolithiasic rats as a preventive agent against the development of kidney stones .
	manualset3
172164	5	413359	7	NULL	NULL	NULL	NULL	preventive agent	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , this current study is aimed to look for an alternative treatment by using Herniaria hirsuta on nephrolithiasic rats as a preventive agent against the development of kidney stones .
	manualset3
172165	6	413359	7	NULL	NULL	NULL	NULL	development	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , this current study is aimed to look for an alternative treatment by using Herniaria hirsuta on nephrolithiasic rats as a preventive agent against the development of kidney stones .
	manualset3
172166	7	413359	7	NULL	NULL	0	NULL	kidney stones	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , this current study is aimed to look for an alternative treatment by using Herniaria hirsuta on nephrolithiasic rats as a preventive agent against the development of kidney stones .
	manualset3
172167	1	413360	7	NULL	NULL	0	NULL	microfluidic/electrochemistry strategy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , this microfluidic/electrochemistry strategy selectively activates the surface for ligand patterning that exactly matches the channel design of the microfluidic channel .
	manualset3
172168	2	413360	7	NULL	NULL	0	NULL	surface	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , this microfluidic/electrochemistry strategy selectively activates the surface for ligand patterning that exactly matches the channel design of the microfluidic channel .
	manualset3
172169	3	413360	7	NULL	NULL	0	NULL	ligand patterning	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , this microfluidic/electrochemistry strategy selectively activates the surface for ligand patterning that exactly matches the channel design of the microfluidic channel .
	manualset3
172170	4	413360	7	NULL	NULL	0	NULL	 channel design	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , this microfluidic/electrochemistry strategy selectively activates the surface for ligand patterning that exactly matches the channel design of the microfluidic channel .
	manualset3
172171	5	413360	7	NULL	NULL	0	NULL	microfluidic channel	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , this microfluidic/electrochemistry strategy selectively activates the surface for ligand patterning that exactly matches the channel design of the microfluidic channel .
	manualset3
172172	1	413361	7	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , this study examined the intercellular transport and protein transduction of the Tat protein .
	manualset3
172173	2	413361	7	NULL	NULL	0	NULL	intercellular transport 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , this study examined the intercellular transport and protein transduction of the Tat protein .
	manualset3
172174	3	413361	7	NULL	NULL	0	NULL	protein transduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , this study examined the intercellular transport and protein transduction of the Tat protein .
	manualset3
172175	4	413361	7	NULL	NULL	0	NULL	Tat protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , this study examined the intercellular transport and protein transduction of the Tat protein .
	manualset3
172176	1	413362	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , this study was aimed at investigating whether HG state could induce OB apoptosis through ONOO - .
	manualset3
172177	2	413362	7	NULL	NULL	0	NULL	HG state	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , this study was aimed at investigating whether HG state could induce OB apoptosis through ONOO - .
	manualset3
172178	3	413362	7	NULL	NULL	0	NULL	OB apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , this study was aimed at investigating whether HG state could induce OB apoptosis through ONOO - .
	manualset3
172179	4	413362	7	NULL	NULL	0	NULL	ONOO -	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , this study was aimed at investigating whether HG state could induce OB apoptosis through ONOO - .
	manualset3
172180	1	413363	7	NULL	NULL	0	NULL	transfection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , transfection of woodchuck livers with recombinant WHV DNA induces active virus replication and gene expression and yields progeny genomes that are faithful copies of the input virus genome .
	manualset3
172181	2	413363	7	NULL	NULL	0	NULL	 woodchuck livers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , transfection of woodchuck livers with recombinant WHV DNA induces active virus replication and gene expression and yields progeny genomes that are faithful copies of the input virus genome .
	manualset3
172182	3	413363	7	NULL	NULL	0	NULL	 recombinant WHV DNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , transfection of woodchuck livers with recombinant WHV DNA induces active virus replication and gene expression and yields progeny genomes that are faithful copies of the input virus genome .
	manualset3
172183	4	413363	7	NULL	NULL	0	NULL	active virus replication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , transfection of woodchuck livers with recombinant WHV DNA induces active virus replication and gene expression and yields progeny genomes that are faithful copies of the input virus genome .
	manualset3
172184	5	413363	7	NULL	NULL	0	NULL	gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , transfection of woodchuck livers with recombinant WHV DNA induces active virus replication and gene expression and yields progeny genomes that are faithful copies of the input virus genome .
	manualset3
172185	6	413363	7	NULL	NULL	NULL	NULL	progeny genomes	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , transfection of woodchuck livers with recombinant WHV DNA induces active virus replication and gene expression and yields progeny genomes that are faithful copies of the input virus genome .
	manualset3
172186	7	413363	7	NULL	NULL	0	NULL	copies	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , transfection of woodchuck livers with recombinant WHV DNA induces active virus replication and gene expression and yields progeny genomes that are faithful copies of the input virus genome .
	manualset3
172187	8	413363	7	NULL	NULL	NULL	NULL	input virus genome	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , transfection of woodchuck livers with recombinant WHV DNA induces active virus replication and gene expression and yields progeny genomes that are faithful copies of the input virus genome .
	manualset3
172188	1	413364	7	NULL	NULL	0	NULL	 two fluorescent dyes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , two fluorescent dyes ( fluorescein and Alexa Fluor 633 ) have been exposed to low-energy proton and alpha radiation with total fluences comparable or exceeding that expected during an unshielded cruise to Mars .
	manualset3
172189	2	413364	7	NULL	NULL	0	NULL	fluorescein	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , two fluorescent dyes ( fluorescein and Alexa Fluor 633 ) have been exposed to low-energy proton and alpha radiation with total fluences comparable or exceeding that expected during an unshielded cruise to Mars .
	manualset3
172190	3	413364	7	NULL	NULL	0	NULL	Alexa Fluor 633	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , two fluorescent dyes ( fluorescein and Alexa Fluor 633 ) have been exposed to low-energy proton and alpha radiation with total fluences comparable or exceeding that expected during an unshielded cruise to Mars .
	manualset3
172191	4	413364	7	NULL	NULL	NULL	NULL	low-energy proton radiation	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , two fluorescent dyes ( fluorescein and Alexa Fluor 633 ) have been exposed to low-energy proton and alpha radiation with total fluences comparable or exceeding that expected during an unshielded cruise to Mars .
	manualset3
172192	5	413364	7	NULL	NULL	0	NULL	unshielded cruise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , two fluorescent dyes ( fluorescein and Alexa Fluor 633 ) have been exposed to low-energy proton and alpha radiation with total fluences comparable or exceeding that expected during an unshielded cruise to Mars .
	manualset3
172193	6	413364	7	NULL	NULL	0	NULL	Mars	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , two fluorescent dyes ( fluorescein and Alexa Fluor 633 ) have been exposed to low-energy proton and alpha radiation with total fluences comparable or exceeding that expected during an unshielded cruise to Mars .
	manualset3
173621	7	413364	7	NULL	NULL	0	NULL	alpha radiation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , two fluorescent dyes ( fluorescein and Alexa Fluor 633 ) have been exposed to low-energy proton and alpha radiation with total fluences comparable or exceeding that expected during an unshielded cruise to Mars .
	manualset3
172194	1	413365	7	NULL	NULL	0	NULL	Acute asthma exacerbations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute asthma exacerbations are one of the most common reasons for paediatric emergency department visits and hospitalisations , and a relapse frequently necessitates repeat urgent care .
	manualset3
172195	2	413365	7	NULL	NULL	0	NULL	reasons	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute asthma exacerbations are one of the most common reasons for paediatric emergency department visits and hospitalisations , and a relapse frequently necessitates repeat urgent care .
	manualset3
172196	3	413365	7	NULL	NULL	NULL	NULL	 paediatric emergency department visits 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Acute asthma exacerbations are one of the most common reasons for paediatric emergency department visits and hospitalisations , and a relapse frequently necessitates repeat urgent care .
	manualset3
172197	4	413365	7	NULL	NULL	0	NULL	hospitalisations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute asthma exacerbations are one of the most common reasons for paediatric emergency department visits and hospitalisations , and a relapse frequently necessitates repeat urgent care .
	manualset3
172198	5	413365	7	NULL	NULL	0	NULL	relapse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute asthma exacerbations are one of the most common reasons for paediatric emergency department visits and hospitalisations , and a relapse frequently necessitates repeat urgent care .
	manualset3
172199	6	413365	7	NULL	NULL	0	NULL	urgent care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute asthma exacerbations are one of the most common reasons for paediatric emergency department visits and hospitalisations , and a relapse frequently necessitates repeat urgent care .
	manualset3
172200	1	413366	7	NULL	NULL	0	NULL	pathogenic mechanisms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , understanding the pathogenic mechanisms of VRE bacteremia is important for prophylaxis .
	manualset3
172201	2	413366	7	NULL	NULL	0	NULL	VRE bacteremia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , understanding the pathogenic mechanisms of VRE bacteremia is important for prophylaxis .
	manualset3
172202	3	413366	7	NULL	NULL	0	NULL	prophylaxis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , understanding the pathogenic mechanisms of VRE bacteremia is important for prophylaxis .
	manualset3
172203	1	413367	7	NULL	NULL	0	NULL	 up-regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , up-regulation of Wee1p alone can not enforce a checkpoint arrest .
	manualset3
172204	2	413367	7	NULL	NULL	0	NULL	Wee1p	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , up-regulation of Wee1p alone can not enforce a checkpoint arrest .
	manualset3
172205	3	413367	7	NULL	NULL	0	NULL	checkpoint arrest	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , up-regulation of Wee1p alone can not enforce a checkpoint arrest .
	manualset3
172206	1	413368	7	NULL	NULL	0	NULL	association	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we also evaluated the association between Mas and the HPA-3 polymorphism .
	manualset3
172207	2	413368	7	NULL	NULL	0	NULL	Mas polymorphism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we also evaluated the association between Mas and the HPA-3 polymorphism .
	manualset3
172208	3	413368	7	NULL	NULL	0	NULL	HPA-3 polymorphism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we also evaluated the association between Mas and the HPA-3 polymorphism .
	manualset3
172209	1	413369	7	NULL	NULL	0	NULL	distribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we analyzed the distribution of Merkel cells in epidermis and dermis of plantar skin of human embryos and fetuses , ranging in gestational age between 7 and 17 weeks .
	manualset3
172210	2	413369	7	NULL	NULL	0	NULL	Merkel cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we analyzed the distribution of Merkel cells in epidermis and dermis of plantar skin of human embryos and fetuses , ranging in gestational age between 7 and 17 weeks .
	manualset3
172211	3	413369	7	NULL	NULL	0	NULL	epidermis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we analyzed the distribution of Merkel cells in epidermis and dermis of plantar skin of human embryos and fetuses , ranging in gestational age between 7 and 17 weeks .
	manualset3
172212	4	413369	7	NULL	NULL	0	NULL	dermis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we analyzed the distribution of Merkel cells in epidermis and dermis of plantar skin of human embryos and fetuses , ranging in gestational age between 7 and 17 weeks .
	manualset3
172213	5	413369	7	NULL	NULL	0	NULL	 plantar skin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we analyzed the distribution of Merkel cells in epidermis and dermis of plantar skin of human embryos and fetuses , ranging in gestational age between 7 and 17 weeks .
	manualset3
172214	6	413369	7	NULL	NULL	0	NULL	human embryos	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we analyzed the distribution of Merkel cells in epidermis and dermis of plantar skin of human embryos and fetuses , ranging in gestational age between 7 and 17 weeks .
	manualset3
172215	7	413369	7	NULL	NULL	0	NULL	 fetuses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we analyzed the distribution of Merkel cells in epidermis and dermis of plantar skin of human embryos and fetuses , ranging in gestational age between 7 and 17 weeks .
	manualset3
172216	8	413369	7	NULL	NULL	NULL	NULL	gestational age	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , we analyzed the distribution of Merkel cells in epidermis and dermis of plantar skin of human embryos and fetuses , ranging in gestational age between 7 and 17 weeks .
	manualset3
172217	9	413369	7	NULL	NULL	0	NULL	7 and 17 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we analyzed the distribution of Merkel cells in epidermis and dermis of plantar skin of human embryos and fetuses , ranging in gestational age between 7 and 17 weeks .
	manualset3
172247	1	413370	7	NULL	NULL	0	NULL	presence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we conclude that the presence of gastrin ( CCK-B ) receptors in the azaserine-induced pancreatic carcinoma DSL-6 , in contrast to their absence in premalignant nodules , suggests that the expression of the gastrin ( CCK-B ) receptor may be important in the transformation from premalignant nodules to pancreatic cancer .
	manualset3
172250	2	413370	7	NULL	NULL	NULL	NULL	gastrin ( CCK-B ) receptors	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , we conclude that the presence of gastrin ( CCK-B ) receptors in the azaserine-induced pancreatic carcinoma DSL-6 , in contrast to their absence in premalignant nodules , suggests that the expression of the gastrin ( CCK-B ) receptor may be important in the transformation from premalignant nodules to pancreatic cancer .
	manualset3
172252	3	413370	7	NULL	NULL	0	NULL	azaserine-induced pancreatic carcinoma DSL-6 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we conclude that the presence of gastrin ( CCK-B ) receptors in the azaserine-induced pancreatic carcinoma DSL-6 , in contrast to their absence in premalignant nodules , suggests that the expression of the gastrin ( CCK-B ) receptor may be important in the transformation from premalignant nodules to pancreatic cancer .
	manualset3
172253	4	413370	7	NULL	NULL	0	NULL	absence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we conclude that the presence of gastrin ( CCK-B ) receptors in the azaserine-induced pancreatic carcinoma DSL-6 , in contrast to their absence in premalignant nodules , suggests that the expression of the gastrin ( CCK-B ) receptor may be important in the transformation from premalignant nodules to pancreatic cancer .
	manualset3
172254	5	413370	7	NULL	NULL	0	NULL	premalignant nodules	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we conclude that the presence of gastrin ( CCK-B ) receptors in the azaserine-induced pancreatic carcinoma DSL-6 , in contrast to their absence in premalignant nodules , suggests that the expression of the gastrin ( CCK-B ) receptor may be important in the transformation from premalignant nodules to pancreatic cancer .
	manualset3
172255	6	413370	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we conclude that the presence of gastrin ( CCK-B ) receptors in the azaserine-induced pancreatic carcinoma DSL-6 , in contrast to their absence in premalignant nodules , suggests that the expression of the gastrin ( CCK-B ) receptor may be important in the transformation from premalignant nodules to pancreatic cancer .
	manualset3
172256	7	413370	7	NULL	NULL	0	NULL	gastrin ( CCK-B ) receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we conclude that the presence of gastrin ( CCK-B ) receptors in the azaserine-induced pancreatic carcinoma DSL-6 , in contrast to their absence in premalignant nodules , suggests that the expression of the gastrin ( CCK-B ) receptor may be important in the transformation from premalignant nodules to pancreatic cancer .
	manualset3
172257	8	413370	7	NULL	NULL	0	NULL	transformation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we conclude that the presence of gastrin ( CCK-B ) receptors in the azaserine-induced pancreatic carcinoma DSL-6 , in contrast to their absence in premalignant nodules , suggests that the expression of the gastrin ( CCK-B ) receptor may be important in the transformation from premalignant nodules to pancreatic cancer .
	manualset3
172258	9	413370	7	NULL	NULL	0	NULL	premalignant nodules	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we conclude that the presence of gastrin ( CCK-B ) receptors in the azaserine-induced pancreatic carcinoma DSL-6 , in contrast to their absence in premalignant nodules , suggests that the expression of the gastrin ( CCK-B ) receptor may be important in the transformation from premalignant nodules to pancreatic cancer .
	manualset3
172259	10	413370	7	NULL	NULL	0	NULL	pancreatic cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we conclude that the presence of gastrin ( CCK-B ) receptors in the azaserine-induced pancreatic carcinoma DSL-6 , in contrast to their absence in premalignant nodules , suggests that the expression of the gastrin ( CCK-B ) receptor may be important in the transformation from premalignant nodules to pancreatic cancer .
	manualset3
172264	1	413371	7	NULL	NULL	0	NULL	key findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we confirmed the key findings by replicating these experiments in human neuroblastoma SK-N-SH cells .
	manualset3
172265	2	413371	7	NULL	NULL	0	NULL	experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we confirmed the key findings by replicating these experiments in human neuroblastoma SK-N-SH cells .
	manualset3
172270	3	413371	7	NULL	NULL	0	NULL	human neuroblastoma SK-N-SH cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we confirmed the key findings by replicating these experiments in human neuroblastoma SK-N-SH cells .
	manualset3
172271	1	413372	7	NULL	NULL	0	NULL	pseudomonas elastase-cleaved Fe-transferrin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we examined whether pseudomonas elastase-cleaved Fe-transferrin and pyocyanin synergistically enhance pulmonary artery endothelial cell injury via .
	manualset3
172272	2	413372	7	NULL	NULL	0	NULL	pyocyanin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we examined whether pseudomonas elastase-cleaved Fe-transferrin and pyocyanin synergistically enhance pulmonary artery endothelial cell injury via .
	manualset3
172273	3	413372	7	NULL	NULL	0	NULL	pulmonary artery endothelial cell injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we examined whether pseudomonas elastase-cleaved Fe-transferrin and pyocyanin synergistically enhance pulmonary artery endothelial cell injury via .
	manualset3
172274	1	413373	7	NULL	NULL	0	NULL	immunoglobulin genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we have constructed immunoglobulin genes in which the DNA segments encoding mouse variable regions specific for the hapten trinitrophenyl ( TNP ) are joined to segments encoding human mu and kappa constant regions .
	manualset3
172275	2	413373	7	NULL	NULL	0	NULL	 DNA segments	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we have constructed immunoglobulin genes in which the DNA segments encoding mouse variable regions specific for the hapten trinitrophenyl ( TNP ) are joined to segments encoding human mu and kappa constant regions .
	manualset3
172276	3	413373	7	NULL	NULL	0	NULL	mouse variable regions	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we have constructed immunoglobulin genes in which the DNA segments encoding mouse variable regions specific for the hapten trinitrophenyl ( TNP ) are joined to segments encoding human mu and kappa constant regions .
	manualset3
172277	4	413373	7	NULL	NULL	0	NULL	hapten trinitrophenyl ( TNP )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we have constructed immunoglobulin genes in which the DNA segments encoding mouse variable regions specific for the hapten trinitrophenyl ( TNP ) are joined to segments encoding human mu and kappa constant regions .
	manualset3
172278	5	413373	7	NULL	NULL	0	NULL	segments 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we have constructed immunoglobulin genes in which the DNA segments encoding mouse variable regions specific for the hapten trinitrophenyl ( TNP ) are joined to segments encoding human mu and kappa constant regions .
	manualset3
172279	6	413373	7	NULL	NULL	0	NULL	human mu constant region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we have constructed immunoglobulin genes in which the DNA segments encoding mouse variable regions specific for the hapten trinitrophenyl ( TNP ) are joined to segments encoding human mu and kappa constant regions .
	manualset3
172280	7	413373	7	NULL	NULL	0	NULL	kappa constant regions 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we have constructed immunoglobulin genes in which the DNA segments encoding mouse variable regions specific for the hapten trinitrophenyl ( TNP ) are joined to segments encoding human mu and kappa constant regions .
	manualset3
172281	1	413374	7	NULL	NULL	0	NULL	Acute care restructuring	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute care restructuring in Newfoundland and Labrador : the history and impact on expenditure .
	manualset3
172282	2	413374	7	NULL	NULL	0	NULL	Newfoundland	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute care restructuring in Newfoundland and Labrador : the history and impact on expenditure .
	manualset3
172283	3	413374	7	NULL	NULL	0	NULL	Labrador	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute care restructuring in Newfoundland and Labrador : the history and impact on expenditure .
	manualset3
172284	4	413374	7	NULL	NULL	0	NULL	history	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute care restructuring in Newfoundland and Labrador : the history and impact on expenditure .
	manualset3
172285	5	413374	7	NULL	NULL	0	NULL	impact 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute care restructuring in Newfoundland and Labrador : the history and impact on expenditure .
	manualset3
172286	6	413374	7	NULL	NULL	0	NULL	expenditure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute care restructuring in Newfoundland and Labrador : the history and impact on expenditure .
	manualset3
172287	1	413375	7	NULL	NULL	0	NULL	new chimeric protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we have expressed and purified a new chimeric protein , hGM-CSF-Bad , linking the human granulocyte-macrophage colony-stimulating factor to the N-terminus of the proapoptotic protein human Bad , to deliver Bad into tumor cells and induce apoptosis .
	manualset3
172288	2	413375	7	NULL	NULL	0	NULL	hGM-CSF-Bad	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we have expressed and purified a new chimeric protein , hGM-CSF-Bad , linking the human granulocyte-macrophage colony-stimulating factor to the N-terminus of the proapoptotic protein human Bad , to deliver Bad into tumor cells and induce apoptosis .
	manualset3
172289	3	413375	7	NULL	NULL	0	NULL	 human granulocyte-macrophage colony-stimulating factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we have expressed and purified a new chimeric protein , hGM-CSF-Bad , linking the human granulocyte-macrophage colony-stimulating factor to the N-terminus of the proapoptotic protein human Bad , to deliver Bad into tumor cells and induce apoptosis .
	manualset3
172290	4	413375	7	NULL	NULL	0	NULL	N-terminus	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we have expressed and purified a new chimeric protein , hGM-CSF-Bad , linking the human granulocyte-macrophage colony-stimulating factor to the N-terminus of the proapoptotic protein human Bad , to deliver Bad into tumor cells and induce apoptosis .
	manualset3
172291	5	413375	7	NULL	NULL	0	NULL	proapoptotic protein human Bad	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we have expressed and purified a new chimeric protein , hGM-CSF-Bad , linking the human granulocyte-macrophage colony-stimulating factor to the N-terminus of the proapoptotic protein human Bad , to deliver Bad into tumor cells and induce apoptosis .
	manualset3
172292	6	413375	7	NULL	NULL	0	NULL	Bad 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we have expressed and purified a new chimeric protein , hGM-CSF-Bad , linking the human granulocyte-macrophage colony-stimulating factor to the N-terminus of the proapoptotic protein human Bad , to deliver Bad into tumor cells and induce apoptosis .
	manualset3
172293	7	413375	7	NULL	NULL	0	NULL	tumor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we have expressed and purified a new chimeric protein , hGM-CSF-Bad , linking the human granulocyte-macrophage colony-stimulating factor to the N-terminus of the proapoptotic protein human Bad , to deliver Bad into tumor cells and induce apoptosis .
	manualset3
172294	8	413375	7	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we have expressed and purified a new chimeric protein , hGM-CSF-Bad , linking the human granulocyte-macrophage colony-stimulating factor to the N-terminus of the proapoptotic protein human Bad , to deliver Bad into tumor cells and induce apoptosis .
	manualset3
172295	1	413376	7	NULL	NULL	0	NULL	influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we have investigated the influence of the TXA2/PGH2 receptor-antagonists , 13-azaprostanoic acid ( 13-APA ) and the BM 13.177 compound , on the formation of thrombi-like platelet aggregates on CI and CIII-coated surfaces .
	manualset3
172296	2	413376	7	NULL	NULL	0	NULL	TXA2/PGH2 receptor-antagonists	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we have investigated the influence of the TXA2/PGH2 receptor-antagonists , 13-azaprostanoic acid ( 13-APA ) and the BM 13.177 compound , on the formation of thrombi-like platelet aggregates on CI and CIII-coated surfaces .
	manualset3
172297	3	413376	7	NULL	NULL	0	NULL	13-azaprostanoic acid ( 13-APA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we have investigated the influence of the TXA2/PGH2 receptor-antagonists , 13-azaprostanoic acid ( 13-APA ) and the BM 13.177 compound , on the formation of thrombi-like platelet aggregates on CI and CIII-coated surfaces .
	manualset3
172298	4	413376	7	NULL	NULL	0	NULL	BM 13.177 compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we have investigated the influence of the TXA2/PGH2 receptor-antagonists , 13-azaprostanoic acid ( 13-APA ) and the BM 13.177 compound , on the formation of thrombi-like platelet aggregates on CI and CIII-coated surfaces .
	manualset3
172299	5	413376	7	NULL	NULL	0	NULL	formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we have investigated the influence of the TXA2/PGH2 receptor-antagonists , 13-azaprostanoic acid ( 13-APA ) and the BM 13.177 compound , on the formation of thrombi-like platelet aggregates on CI and CIII-coated surfaces .
	manualset3
172300	6	413376	7	NULL	NULL	0	NULL	thrombi-like platelet aggregates	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we have investigated the influence of the TXA2/PGH2 receptor-antagonists , 13-azaprostanoic acid ( 13-APA ) and the BM 13.177 compound , on the formation of thrombi-like platelet aggregates on CI and CIII-coated surfaces .
	manualset3
172301	7	413376	7	NULL	NULL	0	NULL	CI and CIII-coated surfaces 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we have investigated the influence of the TXA2/PGH2 receptor-antagonists , 13-azaprostanoic acid ( 13-APA ) and the BM 13.177 compound , on the formation of thrombi-like platelet aggregates on CI and CIII-coated surfaces .
	manualset3
172302	1	413377	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated expression of candidate thyroid hormone transporters L-type amino acid transporter 1 ( Lat1 ) , monocarboxylate transporter ( Mct ) 8 , Mct10 , and organic anion transporting polypeptide 1c1 ( Oatp1c1 ) in mouse cochlear development by in situ hybridization and immunofluorescence analysis .
	manualset3
172303	2	413377	7	NULL	NULL	0	NULL	candidate thyroid hormone transporters L-type amino acid transporter 1 ( Lat1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated expression of candidate thyroid hormone transporters L-type amino acid transporter 1 ( Lat1 ) , monocarboxylate transporter ( Mct ) 8 , Mct10 , and organic anion transporting polypeptide 1c1 ( Oatp1c1 ) in mouse cochlear development by in situ hybridization and immunofluorescence analysis .
	manualset3
172304	3	413377	7	NULL	NULL	0	NULL	monocarboxylate transporter ( Mct ) 8	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated expression of candidate thyroid hormone transporters L-type amino acid transporter 1 ( Lat1 ) , monocarboxylate transporter ( Mct ) 8 , Mct10 , and organic anion transporting polypeptide 1c1 ( Oatp1c1 ) in mouse cochlear development by in situ hybridization and immunofluorescence analysis .
	manualset3
172305	4	413377	7	NULL	NULL	0	NULL	Mct10	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated expression of candidate thyroid hormone transporters L-type amino acid transporter 1 ( Lat1 ) , monocarboxylate transporter ( Mct ) 8 , Mct10 , and organic anion transporting polypeptide 1c1 ( Oatp1c1 ) in mouse cochlear development by in situ hybridization and immunofluorescence analysis .
	manualset3
172306	5	413377	7	NULL	NULL	0	NULL	organic anion transporting polypeptide 1c1 ( Oatp1c1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated expression of candidate thyroid hormone transporters L-type amino acid transporter 1 ( Lat1 ) , monocarboxylate transporter ( Mct ) 8 , Mct10 , and organic anion transporting polypeptide 1c1 ( Oatp1c1 ) in mouse cochlear development by in situ hybridization and immunofluorescence analysis .
	manualset3
172307	6	413377	7	NULL	NULL	0	NULL	mouse cochlear development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated expression of candidate thyroid hormone transporters L-type amino acid transporter 1 ( Lat1 ) , monocarboxylate transporter ( Mct ) 8 , Mct10 , and organic anion transporting polypeptide 1c1 ( Oatp1c1 ) in mouse cochlear development by in situ hybridization and immunofluorescence analysis .
	manualset3
172308	7	413377	7	NULL	NULL	0	NULL	in situ hybridization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated expression of candidate thyroid hormone transporters L-type amino acid transporter 1 ( Lat1 ) , monocarboxylate transporter ( Mct ) 8 , Mct10 , and organic anion transporting polypeptide 1c1 ( Oatp1c1 ) in mouse cochlear development by in situ hybridization and immunofluorescence analysis .
	manualset3
172309	8	413377	7	NULL	NULL	0	NULL	 immunofluorescence analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated expression of candidate thyroid hormone transporters L-type amino acid transporter 1 ( Lat1 ) , monocarboxylate transporter ( Mct ) 8 , Mct10 , and organic anion transporting polypeptide 1c1 ( Oatp1c1 ) in mouse cochlear development by in situ hybridization and immunofluorescence analysis .
	manualset3
172310	1	413378	7	NULL	NULL	0	NULL	repeated microinjections	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated if repeated microinjections of 6-OHDA into the striatum of mice may generate a subchronic model with progressive degeneration .
	manualset3
172311	2	413378	7	NULL	NULL	0	NULL	6-OHDA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated if repeated microinjections of 6-OHDA into the striatum of mice may generate a subchronic model with progressive degeneration .
	manualset3
172312	3	413378	7	NULL	NULL	0	NULL	striatum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated if repeated microinjections of 6-OHDA into the striatum of mice may generate a subchronic model with progressive degeneration .
	manualset3
172313	4	413378	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated if repeated microinjections of 6-OHDA into the striatum of mice may generate a subchronic model with progressive degeneration .
	manualset3
172314	5	413378	7	NULL	NULL	0	NULL	subchronic model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated if repeated microinjections of 6-OHDA into the striatum of mice may generate a subchronic model with progressive degeneration .
	manualset3
172315	6	413378	7	NULL	NULL	0	NULL	progressive degeneration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated if repeated microinjections of 6-OHDA into the striatum of mice may generate a subchronic model with progressive degeneration .
	manualset3
172316	1	413379	7	NULL	NULL	0	NULL	taurine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated the ability of taurine to correct altered islet vascularization .
	manualset3
172317	2	413379	7	NULL	NULL	0	NULL	altered islet vascularization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated the ability of taurine to correct altered islet vascularization .
	manualset3
173622	3	413379	7	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated the ability of taurine to correct altered islet vascularization .
	manualset3
172318	1	413380	7	NULL	NULL	0	NULL	effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated the effects of microinjection of VIP in the dorsal vagal complex ( DVC ) , nucleus raphe obscurus ( nROb ) and nucleus ambiguus of alpha-chloralose-anesthetized rats while recording intragastric pressure , pyloric and greater curvature smooth muscle contractile activity , blood pressure and heart rate .
	manualset3
172319	3	413380	7	NULL	NULL	NULL	NULL	VIP	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated the effects of microinjection of VIP in the dorsal vagal complex ( DVC ) , nucleus raphe obscurus ( nROb ) and nucleus ambiguus of alpha-chloralose-anesthetized rats while recording intragastric pressure , pyloric and greater curvature smooth muscle contractile activity , blood pressure and heart rate .
	manualset3
172320	2	413380	7	NULL	NULL	0	NULL	microinjection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated the effects of microinjection of VIP in the dorsal vagal complex ( DVC ) , nucleus raphe obscurus ( nROb ) and nucleus ambiguus of alpha-chloralose-anesthetized rats while recording intragastric pressure , pyloric and greater curvature smooth muscle contractile activity , blood pressure and heart rate .
	manualset3
172321	4	413380	7	NULL	NULL	0	NULL	dorsal vagal complex ( DVC )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated the effects of microinjection of VIP in the dorsal vagal complex ( DVC ) , nucleus raphe obscurus ( nROb ) and nucleus ambiguus of alpha-chloralose-anesthetized rats while recording intragastric pressure , pyloric and greater curvature smooth muscle contractile activity , blood pressure and heart rate .
	manualset3
172322	5	413380	7	NULL	NULL	NULL	NULL	nucleus raphe obscurus ( nROb )	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated the effects of microinjection of VIP in the dorsal vagal complex ( DVC ) , nucleus raphe obscurus ( nROb ) and nucleus ambiguus of alpha-chloralose-anesthetized rats while recording intragastric pressure , pyloric and greater curvature smooth muscle contractile activity , blood pressure and heart rate .
	manualset3
172323	6	413380	7	NULL	NULL	NULL	NULL	nucleus ambiguus	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated the effects of microinjection of VIP in the dorsal vagal complex ( DVC ) , nucleus raphe obscurus ( nROb ) and nucleus ambiguus of alpha-chloralose-anesthetized rats while recording intragastric pressure , pyloric and greater curvature smooth muscle contractile activity , blood pressure and heart rate .
	manualset3
172324	7	413380	7	NULL	NULL	NULL	NULL	alpha-chloralose-anesthetized rats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated the effects of microinjection of VIP in the dorsal vagal complex ( DVC ) , nucleus raphe obscurus ( nROb ) and nucleus ambiguus of alpha-chloralose-anesthetized rats while recording intragastric pressure , pyloric and greater curvature smooth muscle contractile activity , blood pressure and heart rate .
	manualset3
172325	8	413380	7	NULL	NULL	NULL	NULL	 intragastric pressure 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated the effects of microinjection of VIP in the dorsal vagal complex ( DVC ) , nucleus raphe obscurus ( nROb ) and nucleus ambiguus of alpha-chloralose-anesthetized rats while recording intragastric pressure , pyloric and greater curvature smooth muscle contractile activity , blood pressure and heart rate .
	manualset3
172326	9	413380	7	NULL	NULL	NULL	NULL	pyloric and greater curvature smooth muscle contractile activity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated the effects of microinjection of VIP in the dorsal vagal complex ( DVC ) , nucleus raphe obscurus ( nROb ) and nucleus ambiguus of alpha-chloralose-anesthetized rats while recording intragastric pressure , pyloric and greater curvature smooth muscle contractile activity , blood pressure and heart rate .
	manualset3
172327	10	413380	7	NULL	NULL	NULL	NULL	 blood pressure	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated the effects of microinjection of VIP in the dorsal vagal complex ( DVC ) , nucleus raphe obscurus ( nROb ) and nucleus ambiguus of alpha-chloralose-anesthetized rats while recording intragastric pressure , pyloric and greater curvature smooth muscle contractile activity , blood pressure and heart rate .
	manualset3
172328	11	413380	7	NULL	NULL	NULL	NULL	heart rate	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated the effects of microinjection of VIP in the dorsal vagal complex ( DVC ) , nucleus raphe obscurus ( nROb ) and nucleus ambiguus of alpha-chloralose-anesthetized rats while recording intragastric pressure , pyloric and greater curvature smooth muscle contractile activity , blood pressure and heart rate .
	manualset3
172330	1	413381	7	NULL	NULL	0	NULL	induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated the induction of HO-1 level in host cells , which may exert a beneficial effect to minimize viral replication in SK-N-SH cells .
	manualset3
172332	2	413381	7	NULL	NULL	0	NULL	HO-1 level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated the induction of HO-1 level in host cells , which may exert a beneficial effect to minimize viral replication in SK-N-SH cells .
	manualset3
172333	3	413381	7	NULL	NULL	0	NULL	host cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated the induction of HO-1 level in host cells , which may exert a beneficial effect to minimize viral replication in SK-N-SH cells .
	manualset3
172336	4	413381	7	NULL	NULL	0	NULL	beneficial effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated the induction of HO-1 level in host cells , which may exert a beneficial effect to minimize viral replication in SK-N-SH cells .
	manualset3
172338	5	413381	7	NULL	NULL	0	NULL	viral replication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated the induction of HO-1 level in host cells , which may exert a beneficial effect to minimize viral replication in SK-N-SH cells .
	manualset3
172340	6	413381	7	NULL	NULL	0	NULL	SK-N-SH cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we investigated the induction of HO-1 level in host cells , which may exert a beneficial effect to minimize viral replication in SK-N-SH cells .
	manualset3
172342	1	413382	7	NULL	NULL	0	NULL	curative operation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we performed a curative operation with complete D2 lymph node dissection and 16b1 lateral lymph node dissection .
	manualset3
172343	2	413382	7	NULL	NULL	0	NULL	complete D2 lymph node dissection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we performed a curative operation with complete D2 lymph node dissection and 16b1 lateral lymph node dissection .
	manualset3
172344	3	413382	7	NULL	NULL	0	NULL	16b1 lateral lymph node dissection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we performed a curative operation with complete D2 lymph node dissection and 16b1 lateral lymph node dissection .
	manualset3
172357	1	413383	7	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we propose that there are three distinct isoforms of CKII within HeLa cells with different catalytic subunit stoichiometries ( alpha 2 beta 2 , alpha alpha ' beta 2 , and alpha ' 2 beta 2 ) .
	manualset3
172358	2	413383	7	NULL	NULL	0	NULL	isoforms of CKII	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we propose that there are three distinct isoforms of CKII within HeLa cells with different catalytic subunit stoichiometries ( alpha 2 beta 2 , alpha alpha ' beta 2 , and alpha ' 2 beta 2 ) .
	manualset3
172359	3	413383	7	NULL	NULL	0	NULL	HeLa cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we propose that there are three distinct isoforms of CKII within HeLa cells with different catalytic subunit stoichiometries ( alpha 2 beta 2 , alpha alpha ' beta 2 , and alpha ' 2 beta 2 ) .
	manualset3
172360	4	413383	7	NULL	NULL	0	NULL	catalytic subunit stoichiometries	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we propose that there are three distinct isoforms of CKII within HeLa cells with different catalytic subunit stoichiometries ( alpha 2 beta 2 , alpha alpha ' beta 2 , and alpha ' 2 beta 2 ) .
	manualset3
172361	5	413383	7	NULL	NULL	0	NULL	alpha 2 beta 2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we propose that there are three distinct isoforms of CKII within HeLa cells with different catalytic subunit stoichiometries ( alpha 2 beta 2 , alpha alpha ' beta 2 , and alpha ' 2 beta 2 ) .
	manualset3
172362	6	413383	7	NULL	NULL	0	NULL	alpha alpha ' beta 2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we propose that there are three distinct isoforms of CKII within HeLa cells with different catalytic subunit stoichiometries ( alpha 2 beta 2 , alpha alpha ' beta 2 , and alpha ' 2 beta 2 ) .
	manualset3
172363	7	413383	7	NULL	NULL	0	NULL	alpha ' 2 beta 2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we propose that there are three distinct isoforms of CKII within HeLa cells with different catalytic subunit stoichiometries ( alpha 2 beta 2 , alpha alpha ' beta 2 , and alpha ' 2 beta 2 ) .
	manualset3
172364	1	413384	7	NULL	NULL	0	NULL	Acute cessation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute cessation of impulse flow in the habenulo-raph tract also prevented the depamide-induced diminution of cerebral 5-HTP accumulation .
	manualset3
172365	2	413384	7	NULL	NULL	0	NULL	impulse flow	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute cessation of impulse flow in the habenulo-raph tract also prevented the depamide-induced diminution of cerebral 5-HTP accumulation .
	manualset3
172366	3	413384	7	NULL	NULL	0	NULL	habenulo-raph tract 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute cessation of impulse flow in the habenulo-raph tract also prevented the depamide-induced diminution of cerebral 5-HTP accumulation .
	manualset3
172370	4	413384	7	NULL	NULL	0	NULL	depamide-induced diminution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute cessation of impulse flow in the habenulo-raph tract also prevented the depamide-induced diminution of cerebral 5-HTP accumulation .
	manualset3
172372	5	413384	7	NULL	NULL	0	NULL	cerebral 5-HTP accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute cessation of impulse flow in the habenulo-raph tract also prevented the depamide-induced diminution of cerebral 5-HTP accumulation .
	manualset3
172386	1	413385	7	NULL	NULL	0	NULL	view	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we should broaden our view of Beclin1 as a specialized molecule in autophagy to that of a multifunctional protein .
	manualset3
172387	2	413385	7	NULL	NULL	0	NULL	Beclin1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we should broaden our view of Beclin1 as a specialized molecule in autophagy to that of a multifunctional protein .
	manualset3
172388	3	413385	7	NULL	NULL	0	NULL	molecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we should broaden our view of Beclin1 as a specialized molecule in autophagy to that of a multifunctional protein .
	manualset3
172389	4	413385	7	NULL	NULL	0	NULL	autophagy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we should broaden our view of Beclin1 as a specialized molecule in autophagy to that of a multifunctional protein .
	manualset3
172390	5	413385	7	NULL	NULL	0	NULL	multifunctional protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we should broaden our view of Beclin1 as a specialized molecule in autophagy to that of a multifunctional protein .
	manualset3
172391	1	413386	7	NULL	NULL	0	NULL	AR polymorphism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we studied whether AR polymorphism affects bone mineral density , bone mineral density change , or fracture risk in a 5-year randomized hormone replacement therapy ( HRT ) trial on 331 early postmenopausal women ( mean baseline age , 52.7 + / - 2.3 years ) .
	manualset3
172392	2	413386	7	NULL	NULL	0	NULL	bone mineral density	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we studied whether AR polymorphism affects bone mineral density , bone mineral density change , or fracture risk in a 5-year randomized hormone replacement therapy ( HRT ) trial on 331 early postmenopausal women ( mean baseline age , 52.7 + / - 2.3 years ) .
	manualset3
172393	3	413386	7	NULL	NULL	0	NULL	bone mineral density change	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we studied whether AR polymorphism affects bone mineral density , bone mineral density change , or fracture risk in a 5-year randomized hormone replacement therapy ( HRT ) trial on 331 early postmenopausal women ( mean baseline age , 52.7 + / - 2.3 years ) .
	manualset3
172394	4	413386	7	NULL	NULL	0	NULL	fracture risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we studied whether AR polymorphism affects bone mineral density , bone mineral density change , or fracture risk in a 5-year randomized hormone replacement therapy ( HRT ) trial on 331 early postmenopausal women ( mean baseline age , 52.7 + / - 2.3 years ) .
	manualset3
172395	5	413386	7	NULL	NULL	0	NULL	5-year randomized hormone replacement therapy ( HRT ) trial	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we studied whether AR polymorphism affects bone mineral density , bone mineral density change , or fracture risk in a 5-year randomized hormone replacement therapy ( HRT ) trial on 331 early postmenopausal women ( mean baseline age , 52.7 + / - 2.3 years ) .
	manualset3
172396	6	413386	7	NULL	NULL	0	NULL	331	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we studied whether AR polymorphism affects bone mineral density , bone mineral density change , or fracture risk in a 5-year randomized hormone replacement therapy ( HRT ) trial on 331 early postmenopausal women ( mean baseline age , 52.7 + / - 2.3 years ) .
	manualset3
172397	7	413386	7	NULL	NULL	0	NULL	early postmenopausal women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we studied whether AR polymorphism affects bone mineral density , bone mineral density change , or fracture risk in a 5-year randomized hormone replacement therapy ( HRT ) trial on 331 early postmenopausal women ( mean baseline age , 52.7 + / - 2.3 years ) .
	manualset3
172398	8	413386	7	NULL	NULL	0	NULL	mean baseline age 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we studied whether AR polymorphism affects bone mineral density , bone mineral density change , or fracture risk in a 5-year randomized hormone replacement therapy ( HRT ) trial on 331 early postmenopausal women ( mean baseline age , 52.7 + / - 2.3 years ) .
	manualset3
172399	9	413386	7	NULL	NULL	NULL	NULL	52.7 + / - 2.3 years 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , we studied whether AR polymorphism affects bone mineral density , bone mineral density change , or fracture risk in a 5-year randomized hormone replacement therapy ( HRT ) trial on 331 early postmenopausal women ( mean baseline age , 52.7 + / - 2.3 years ) .
	manualset3
172400	1	413387	7	NULL	NULL	0	NULL	markers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we tested if markers in MTHFR ( 5 , 10-methylenetetrahydrofolate reductase ) and RFC1 ( reduced folate carrier 1 ) were associated with oral clefts , depending on the maternal origin defined by the mitochondrial haplotype .
	manualset3
172401	2	413387	7	NULL	NULL	0	NULL	MTHFR ( 5 , 10-methylenetetrahydrofolate reductase )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we tested if markers in MTHFR ( 5 , 10-methylenetetrahydrofolate reductase ) and RFC1 ( reduced folate carrier 1 ) were associated with oral clefts , depending on the maternal origin defined by the mitochondrial haplotype .
	manualset3
172402	3	413387	7	NULL	NULL	0	NULL	RFC1 ( reduced folate carrier 1 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we tested if markers in MTHFR ( 5 , 10-methylenetetrahydrofolate reductase ) and RFC1 ( reduced folate carrier 1 ) were associated with oral clefts , depending on the maternal origin defined by the mitochondrial haplotype .
	manualset3
172403	4	413387	7	NULL	NULL	0	NULL	oral clefts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we tested if markers in MTHFR ( 5 , 10-methylenetetrahydrofolate reductase ) and RFC1 ( reduced folate carrier 1 ) were associated with oral clefts , depending on the maternal origin defined by the mitochondrial haplotype .
	manualset3
172404	5	413387	7	NULL	NULL	0	NULL	maternal origin	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we tested if markers in MTHFR ( 5 , 10-methylenetetrahydrofolate reductase ) and RFC1 ( reduced folate carrier 1 ) were associated with oral clefts , depending on the maternal origin defined by the mitochondrial haplotype .
	manualset3
172405	6	413387	7	NULL	NULL	0	NULL	mitochondrial haplotype	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we tested if markers in MTHFR ( 5 , 10-methylenetetrahydrofolate reductase ) and RFC1 ( reduced folate carrier 1 ) were associated with oral clefts , depending on the maternal origin defined by the mitochondrial haplotype .
	manualset3
172406	1	413388	7	NULL	NULL	NULL	NULL	cardioprotective effect	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , while not compromising the cardioprotective effect of antiplatelet agents , the gastroprotective benefit of PPI should be strongly considered in patients who need both .
	manualset3
172407	2	413388	7	NULL	NULL	0	NULL	antiplatelet agents	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , while not compromising the cardioprotective effect of antiplatelet agents , the gastroprotective benefit of PPI should be strongly considered in patients who need both .
	manualset3
172408	3	413388	7	NULL	NULL	0	NULL	gastroprotective benefit	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , while not compromising the cardioprotective effect of antiplatelet agents , the gastroprotective benefit of PPI should be strongly considered in patients who need both .
	manualset3
172409	4	413388	7	NULL	NULL	0	NULL	PPI	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , while not compromising the cardioprotective effect of antiplatelet agents , the gastroprotective benefit of PPI should be strongly considered in patients who need both .
	manualset3
172410	5	413388	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , while not compromising the cardioprotective effect of antiplatelet agents , the gastroprotective benefit of PPI should be strongly considered in patients who need both .
	manualset3
172411	1	413389	7	NULL	NULL	0	NULL	community staff	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore community staff need to adopt a risk assessment approach and strategies to ensure that adequate decontamination of their hands is achieved in order that care can be given with the minimal risk of cross-infection between patients , clients and staff .
	manualset3
172412	2	413389	7	NULL	NULL	0	NULL	risk assessment approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore community staff need to adopt a risk assessment approach and strategies to ensure that adequate decontamination of their hands is achieved in order that care can be given with the minimal risk of cross-infection between patients , clients and staff .
	manualset3
172413	3	413389	7	NULL	NULL	0	NULL	strategies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore community staff need to adopt a risk assessment approach and strategies to ensure that adequate decontamination of their hands is achieved in order that care can be given with the minimal risk of cross-infection between patients , clients and staff .
	manualset3
172414	4	413389	7	NULL	NULL	0	NULL	adequate decontamination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore community staff need to adopt a risk assessment approach and strategies to ensure that adequate decontamination of their hands is achieved in order that care can be given with the minimal risk of cross-infection between patients , clients and staff .
	manualset3
172415	5	413389	7	NULL	NULL	0	NULL	hands	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore community staff need to adopt a risk assessment approach and strategies to ensure that adequate decontamination of their hands is achieved in order that care can be given with the minimal risk of cross-infection between patients , clients and staff .
	manualset3
172416	6	413389	7	NULL	NULL	0	NULL	care 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore community staff need to adopt a risk assessment approach and strategies to ensure that adequate decontamination of their hands is achieved in order that care can be given with the minimal risk of cross-infection between patients , clients and staff .
	manualset3
172417	7	413389	7	NULL	NULL	0	NULL	minimal risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore community staff need to adopt a risk assessment approach and strategies to ensure that adequate decontamination of their hands is achieved in order that care can be given with the minimal risk of cross-infection between patients , clients and staff .
	manualset3
172418	8	413389	7	NULL	NULL	0	NULL	 cross-infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore community staff need to adopt a risk assessment approach and strategies to ensure that adequate decontamination of their hands is achieved in order that care can be given with the minimal risk of cross-infection between patients , clients and staff .
	manualset3
172419	9	413389	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore community staff need to adopt a risk assessment approach and strategies to ensure that adequate decontamination of their hands is achieved in order that care can be given with the minimal risk of cross-infection between patients , clients and staff .
	manualset3
172420	10	413389	7	NULL	NULL	0	NULL	clients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore community staff need to adopt a risk assessment approach and strategies to ensure that adequate decontamination of their hands is achieved in order that care can be given with the minimal risk of cross-infection between patients , clients and staff .
	manualset3
172421	11	413389	7	NULL	NULL	0	NULL	staff	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore community staff need to adopt a risk assessment approach and strategies to ensure that adequate decontamination of their hands is achieved in order that care can be given with the minimal risk of cross-infection between patients , clients and staff .
	manualset3
172422	1	413390	7	NULL	NULL	0	NULL	 diagnostic manuals	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore diagnostic manuals , like the DSM-IV and the ICD-10 are subjected to changing knowledge derived from research on one hand and to changes of clinical necessities .
	manualset3
172423	2	413390	7	NULL	NULL	0	NULL	DSM-IV	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore diagnostic manuals , like the DSM-IV and the ICD-10 are subjected to changing knowledge derived from research on one hand and to changes of clinical necessities .
	manualset3
172424	3	413390	7	NULL	NULL	0	NULL	ICD-10	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore diagnostic manuals , like the DSM-IV and the ICD-10 are subjected to changing knowledge derived from research on one hand and to changes of clinical necessities .
	manualset3
172425	4	413390	7	NULL	NULL	0	NULL	knowledge	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore diagnostic manuals , like the DSM-IV and the ICD-10 are subjected to changing knowledge derived from research on one hand and to changes of clinical necessities .
	manualset3
172426	5	413390	7	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore diagnostic manuals , like the DSM-IV and the ICD-10 are subjected to changing knowledge derived from research on one hand and to changes of clinical necessities .
	manualset3
172427	7	413390	7	NULL	NULL	NULL	NULL	clinical necessities	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore diagnostic manuals , like the DSM-IV and the ICD-10 are subjected to changing knowledge derived from research on one hand and to changes of clinical necessities .
	manualset3
172698	6	413390	7	NULL	NULL	0	NULL	changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore diagnostic manuals , like the DSM-IV and the ICD-10 are subjected to changing knowledge derived from research on one hand and to changes of clinical necessities .
	manualset3
172428	1	413391	7	NULL	NULL	NULL	NULL	aim 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore the aim of this study was to collect data on the usefulness of results obtained after aerobic culture ( sheepblood , brilliantgreen , sabouraud 's agar ) of swabs and tracheal lavages following standardized sampling .
	manualset3
172429	2	413391	7	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore the aim of this study was to collect data on the usefulness of results obtained after aerobic culture ( sheepblood , brilliantgreen , sabouraud 's agar ) of swabs and tracheal lavages following standardized sampling .
	manualset3
172430	3	413391	7	NULL	NULL	0	NULL	 data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore the aim of this study was to collect data on the usefulness of results obtained after aerobic culture ( sheepblood , brilliantgreen , sabouraud 's agar ) of swabs and tracheal lavages following standardized sampling .
	manualset3
172431	4	413391	7	NULL	NULL	0	NULL	usefulness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore the aim of this study was to collect data on the usefulness of results obtained after aerobic culture ( sheepblood , brilliantgreen , sabouraud 's agar ) of swabs and tracheal lavages following standardized sampling .
	manualset3
172432	5	413391	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore the aim of this study was to collect data on the usefulness of results obtained after aerobic culture ( sheepblood , brilliantgreen , sabouraud 's agar ) of swabs and tracheal lavages following standardized sampling .
	manualset3
172433	6	413391	7	NULL	NULL	0	NULL	aerobic culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore the aim of this study was to collect data on the usefulness of results obtained after aerobic culture ( sheepblood , brilliantgreen , sabouraud 's agar ) of swabs and tracheal lavages following standardized sampling .
	manualset3
172434	7	413391	7	NULL	NULL	NULL	NULL	sheepblood	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore the aim of this study was to collect data on the usefulness of results obtained after aerobic culture ( sheepblood , brilliantgreen , sabouraud 's agar ) of swabs and tracheal lavages following standardized sampling .
	manualset3
172435	8	413391	7	NULL	NULL	0	NULL	brilliantgreen 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore the aim of this study was to collect data on the usefulness of results obtained after aerobic culture ( sheepblood , brilliantgreen , sabouraud 's agar ) of swabs and tracheal lavages following standardized sampling .
	manualset3
172436	9	413391	7	NULL	NULL	0	NULL	sabouraud 's agar	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore the aim of this study was to collect data on the usefulness of results obtained after aerobic culture ( sheepblood , brilliantgreen , sabouraud 's agar ) of swabs and tracheal lavages following standardized sampling .
	manualset3
172437	10	413391	7	NULL	NULL	0	NULL	swabs	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore the aim of this study was to collect data on the usefulness of results obtained after aerobic culture ( sheepblood , brilliantgreen , sabouraud 's agar ) of swabs and tracheal lavages following standardized sampling .
	manualset3
172438	11	413391	7	NULL	NULL	0	NULL	tracheal lavages 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore the aim of this study was to collect data on the usefulness of results obtained after aerobic culture ( sheepblood , brilliantgreen , sabouraud 's agar ) of swabs and tracheal lavages following standardized sampling .
	manualset3
172439	12	413391	7	NULL	NULL	0	NULL	 standardized sampling 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore the aim of this study was to collect data on the usefulness of results obtained after aerobic culture ( sheepblood , brilliantgreen , sabouraud 's agar ) of swabs and tracheal lavages following standardized sampling .
	manualset3
172440	1	413392	7	NULL	NULL	0	NULL	Comparative capillaroscopic study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative capillaroscopic study of certain bioflavonoids and total triterpenic fractions of Centella asiatica in venous insufficiency ) .
	manualset3
172441	2	413392	7	NULL	NULL	0	NULL	bioflavonoids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative capillaroscopic study of certain bioflavonoids and total triterpenic fractions of Centella asiatica in venous insufficiency ) .
	manualset3
172442	3	413392	7	NULL	NULL	0	NULL	total triterpenic fractions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative capillaroscopic study of certain bioflavonoids and total triterpenic fractions of Centella asiatica in venous insufficiency ) .
	manualset3
172443	4	413392	7	NULL	NULL	0	NULL	Centella asiatica	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative capillaroscopic study of certain bioflavonoids and total triterpenic fractions of Centella asiatica in venous insufficiency ) .
	manualset3
172444	5	413392	7	NULL	NULL	0	NULL	venous insufficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative capillaroscopic study of certain bioflavonoids and total triterpenic fractions of Centella asiatica in venous insufficiency ) .
	manualset3
172445	1	413393	7	NULL	NULL	0	NULL	 laboratory information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore we opened the laboratory information and consulting office ( called Kensa Yorozu Consulting Room ) from April , 2004 .
	manualset3
172446	2	413393	7	NULL	NULL	NULL	NULL	consulting office	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore we opened the laboratory information and consulting office ( called Kensa Yorozu Consulting Room ) from April , 2004 .
	manualset3
172447	3	413393	7	NULL	NULL	NULL	NULL	Kensa Yorozu Consulting Room	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore we opened the laboratory information and consulting office ( called Kensa Yorozu Consulting Room ) from April , 2004 .
	manualset3
172448	4	413393	7	NULL	NULL	0	NULL	April , 2004	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore we opened the laboratory information and consulting office ( called Kensa Yorozu Consulting Room ) from April , 2004 .
	manualset3
172449	1	413394	7	NULL	NULL	0	NULL	Thermal denaturation midpoint temperatures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermal denaturation midpoint temperatures of recombinant oleosins were also assayed and found to be very similar to that of native oleosins , indicating proper structural conformation of the recombinant proteins .
	manualset3
172450	2	413394	7	NULL	NULL	0	NULL	recombinant oleosins	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermal denaturation midpoint temperatures of recombinant oleosins were also assayed and found to be very similar to that of native oleosins , indicating proper structural conformation of the recombinant proteins .
	manualset3
172452	3	413394	7	NULL	NULL	0	NULL	 native oleosins	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermal denaturation midpoint temperatures of recombinant oleosins were also assayed and found to be very similar to that of native oleosins , indicating proper structural conformation of the recombinant proteins .
	manualset3
172453	4	413394	7	NULL	NULL	0	NULL	proper structural conformation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermal denaturation midpoint temperatures of recombinant oleosins were also assayed and found to be very similar to that of native oleosins , indicating proper structural conformation of the recombinant proteins .
	manualset3
172454	5	413394	7	NULL	NULL	0	NULL	recombinant proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermal denaturation midpoint temperatures of recombinant oleosins were also assayed and found to be very similar to that of native oleosins , indicating proper structural conformation of the recombinant proteins .
	manualset3
172455	1	413395	7	NULL	NULL	0	NULL	Thermal hysteresis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermal hysteresis in the backbone and side-chain dynamics of the elastin mimetic peptide ( VPGVG ) 3 revealed by 2H NMR .
	manualset3
172456	2	413395	7	NULL	NULL	0	NULL	 backbone	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermal hysteresis in the backbone and side-chain dynamics of the elastin mimetic peptide ( VPGVG ) 3 revealed by 2H NMR .
	manualset3
172457	3	413395	7	NULL	NULL	0	NULL	side-chain dynamics	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermal hysteresis in the backbone and side-chain dynamics of the elastin mimetic peptide ( VPGVG ) 3 revealed by 2H NMR .
	manualset3
172458	4	413395	7	NULL	NULL	0	NULL	elastin mimetic peptide ( VPGVG ) 3	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermal hysteresis in the backbone and side-chain dynamics of the elastin mimetic peptide ( VPGVG ) 3 revealed by 2H NMR .
	manualset3
172459	5	413395	7	NULL	NULL	0	NULL	2H NMR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermal hysteresis in the backbone and side-chain dynamics of the elastin mimetic peptide ( VPGVG ) 3 revealed by 2H NMR .
	manualset3
172460	1	413396	7	NULL	NULL	0	NULL	Thermal lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermal lesions in the ciliary processes were induced with 0.7-second , 1200-mW , and 100 - to 500-microns applications , 0.5 mm from the surgical limbus and defocused 1 mm posteriorly .
	manualset3
172461	2	413396	7	NULL	NULL	0	NULL	ciliary processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermal lesions in the ciliary processes were induced with 0.7-second , 1200-mW , and 100 - to 500-microns applications , 0.5 mm from the surgical limbus and defocused 1 mm posteriorly .
	manualset3
172462	3	413396	7	NULL	NULL	0	NULL	0.7-second 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermal lesions in the ciliary processes were induced with 0.7-second , 1200-mW , and 100 - to 500-microns applications , 0.5 mm from the surgical limbus and defocused 1 mm posteriorly .
	manualset3
172463	4	413396	7	NULL	NULL	0	NULL	1200-mW	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermal lesions in the ciliary processes were induced with 0.7-second , 1200-mW , and 100 - to 500-microns applications , 0.5 mm from the surgical limbus and defocused 1 mm posteriorly .
	manualset3
172464	5	413396	7	NULL	NULL	0	NULL	100 - to 500-microns applications	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermal lesions in the ciliary processes were induced with 0.7-second , 1200-mW , and 100 - to 500-microns applications , 0.5 mm from the surgical limbus and defocused 1 mm posteriorly .
	manualset3
172465	6	413396	7	NULL	NULL	0	NULL	 0.5 mm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermal lesions in the ciliary processes were induced with 0.7-second , 1200-mW , and 100 - to 500-microns applications , 0.5 mm from the surgical limbus and defocused 1 mm posteriorly .
	manualset3
172466	7	413396	7	NULL	NULL	0	NULL	surgical limbus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermal lesions in the ciliary processes were induced with 0.7-second , 1200-mW , and 100 - to 500-microns applications , 0.5 mm from the surgical limbus and defocused 1 mm posteriorly .
	manualset3
172467	8	413396	7	NULL	NULL	0	NULL	1 mm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermal lesions in the ciliary processes were induced with 0.7-second , 1200-mW , and 100 - to 500-microns applications , 0.5 mm from the surgical limbus and defocused 1 mm posteriorly .
	manualset3
172468	1	413397	7	NULL	NULL	0	NULL	Thermally-triggered ` off-on-off ' response	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermally-triggered ` off-on-off ' response of gadolinium-hydrogel-lipid hybrid nanoparticles defines a customizable temperature window for non-invasive magnetic resonance imaging thermometry .
	manualset3
172469	2	413397	7	NULL	NULL	0	NULL	gadolinium-hydrogel-lipid hybrid nanoparticles	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermally-triggered ` off-on-off ' response of gadolinium-hydrogel-lipid hybrid nanoparticles defines a customizable temperature window for non-invasive magnetic resonance imaging thermometry .
	manualset3
172470	3	413397	7	NULL	NULL	0	NULL	 customizable temperature window	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermally-triggered ` off-on-off ' response of gadolinium-hydrogel-lipid hybrid nanoparticles defines a customizable temperature window for non-invasive magnetic resonance imaging thermometry .
	manualset3
172471	4	413397	7	NULL	NULL	0	NULL	non-invasive magnetic resonance imaging thermometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermally-triggered ` off-on-off ' response of gadolinium-hydrogel-lipid hybrid nanoparticles defines a customizable temperature window for non-invasive magnetic resonance imaging thermometry .
	manualset3
172472	1	413398	7	NULL	NULL	0	NULL	Thermoalkalophilic esterase enzyme 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermoalkalophilic esterase enzyme from Balova ( Agamemnon ) geothermal site were aimed to be immobilized effectively via a simple and cost-effective protocol in silicate coated Calcium alginate ( Ca-alginate ) beads by entrapment .
	manualset3
172473	2	413398	7	NULL	NULL	0	NULL	Balova ( Agamemnon ) geothermal site	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermoalkalophilic esterase enzyme from Balova ( Agamemnon ) geothermal site were aimed to be immobilized effectively via a simple and cost-effective protocol in silicate coated Calcium alginate ( Ca-alginate ) beads by entrapment .
	manualset3
172474	3	413398	7	NULL	NULL	0	NULL	simple and cost-effective protocol	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermoalkalophilic esterase enzyme from Balova ( Agamemnon ) geothermal site were aimed to be immobilized effectively via a simple and cost-effective protocol in silicate coated Calcium alginate ( Ca-alginate ) beads by entrapment .
	manualset3
172475	4	413398	7	NULL	NULL	0	NULL	silicate coated Calcium alginate ( Ca-alginate ) beads	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermoalkalophilic esterase enzyme from Balova ( Agamemnon ) geothermal site were aimed to be immobilized effectively via a simple and cost-effective protocol in silicate coated Calcium alginate ( Ca-alginate ) beads by entrapment .
	manualset3
172476	5	413398	7	NULL	NULL	0	NULL	entrapment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermoalkalophilic esterase enzyme from Balova ( Agamemnon ) geothermal site were aimed to be immobilized effectively via a simple and cost-effective protocol in silicate coated Calcium alginate ( Ca-alginate ) beads by entrapment .
	manualset3
172504	1	413399	7	NULL	NULL	NULL	NULL	Thermodynamics	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Thermodynamics for 10 sequences with a GTG bulge were determined to test the applicability of the nearest-neighbor model to a single-bulge loop .
	manualset3
172505	2	413399	7	NULL	NULL	NULL	NULL	10 sequences	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Thermodynamics for 10 sequences with a GTG bulge were determined to test the applicability of the nearest-neighbor model to a single-bulge loop .
	manualset3
172506	3	413399	7	NULL	NULL	NULL	NULL	GTG bulge	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Thermodynamics for 10 sequences with a GTG bulge were determined to test the applicability of the nearest-neighbor model to a single-bulge loop .
	manualset3
172507	4	413399	7	NULL	NULL	0	NULL	applicability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermodynamics for 10 sequences with a GTG bulge were determined to test the applicability of the nearest-neighbor model to a single-bulge loop .
	manualset3
172508	5	413399	7	NULL	NULL	0	NULL	nearest-neighbor model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermodynamics for 10 sequences with a GTG bulge were determined to test the applicability of the nearest-neighbor model to a single-bulge loop .
	manualset3
172509	6	413399	7	NULL	NULL	NULL	NULL	single-bulge loop	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Thermodynamics for 10 sequences with a GTG bulge were determined to test the applicability of the nearest-neighbor model to a single-bulge loop .
	manualset3
172510	1	413400	7	NULL	NULL	0	NULL	Thermodynamics	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermodynamics of left-handed helix formation .
	manualset3
172511	2	413400	7	NULL	NULL	0	NULL	left-handed helix formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermodynamics of left-handed helix formation .
	manualset3
172512	1	413401	7	NULL	NULL	0	NULL	Acute effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute effects of dietary cholic acid and methylazoxymethanol acetate on colon epithelial cell proliferation ; metabolism of bile salts and neutral sterols in conventional and germfree SD rats .
	manualset3
172513	2	413401	7	NULL	NULL	0	NULL	dietary cholic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute effects of dietary cholic acid and methylazoxymethanol acetate on colon epithelial cell proliferation ; metabolism of bile salts and neutral sterols in conventional and germfree SD rats .
	manualset3
172514	3	413401	7	NULL	NULL	0	NULL	methylazoxymethanol acetate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute effects of dietary cholic acid and methylazoxymethanol acetate on colon epithelial cell proliferation ; metabolism of bile salts and neutral sterols in conventional and germfree SD rats .
	manualset3
172515	4	413401	7	NULL	NULL	0	NULL	colon epithelial cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute effects of dietary cholic acid and methylazoxymethanol acetate on colon epithelial cell proliferation ; metabolism of bile salts and neutral sterols in conventional and germfree SD rats .
	manualset3
172516	5	413401	7	NULL	NULL	0	NULL	metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute effects of dietary cholic acid and methylazoxymethanol acetate on colon epithelial cell proliferation ; metabolism of bile salts and neutral sterols in conventional and germfree SD rats .
	manualset3
172517	6	413401	7	NULL	NULL	0	NULL	bile salts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute effects of dietary cholic acid and methylazoxymethanol acetate on colon epithelial cell proliferation ; metabolism of bile salts and neutral sterols in conventional and germfree SD rats .
	manualset3
172518	7	413401	7	NULL	NULL	0	NULL	neutral sterols	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute effects of dietary cholic acid and methylazoxymethanol acetate on colon epithelial cell proliferation ; metabolism of bile salts and neutral sterols in conventional and germfree SD rats .
	manualset3
172519	8	413401	7	NULL	NULL	0	NULL	germfree SD rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute effects of dietary cholic acid and methylazoxymethanol acetate on colon epithelial cell proliferation ; metabolism of bile salts and neutral sterols in conventional and germfree SD rats .
	manualset3
172520	1	413402	7	NULL	NULL	0	NULL	Thermogelling behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermogelling behavior of the aliphatically modified polymer was dependent on the degree of aliphatic modification and polymer concentration .
	manualset3
172521	2	413402	7	NULL	NULL	0	NULL	aliphatically modified polymer	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermogelling behavior of the aliphatically modified polymer was dependent on the degree of aliphatic modification and polymer concentration .
	manualset3
172522	3	413402	7	NULL	NULL	0	NULL	degree	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermogelling behavior of the aliphatically modified polymer was dependent on the degree of aliphatic modification and polymer concentration .
	manualset3
172523	4	413402	7	NULL	NULL	0	NULL	aliphatic modification	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermogelling behavior of the aliphatically modified polymer was dependent on the degree of aliphatic modification and polymer concentration .
	manualset3
172524	5	413402	7	NULL	NULL	0	NULL	polymer concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermogelling behavior of the aliphatically modified polymer was dependent on the degree of aliphatic modification and polymer concentration .
	manualset3
172525	1	413403	7	NULL	NULL	0	NULL	Thermolysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermolysis of 3 , 4-cis ring-fused 5-spirocyclopropane isoxazolidines 16 , 18-21 , 33 , 34 , 38a , and 61 , in the presence of a protic acid at 70-110 degrees C , yielded 3 , 4-cis ring-fused azetidin-2-ones 22-26 , 41 , 42 , 46 , and 62 with concomitant extrusion of ethylene , in good yields .
	manualset3
172526	2	413403	7	NULL	NULL	0	NULL	3 , 4-cis ring-fused 5-spirocyclopropane isoxazolidines 16 , 18-21 , 33 , 34 , 38a , and 61	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermolysis of 3 , 4-cis ring-fused 5-spirocyclopropane isoxazolidines 16 , 18-21 , 33 , 34 , 38a , and 61 , in the presence of a protic acid at 70-110 degrees C , yielded 3 , 4-cis ring-fused azetidin-2-ones 22-26 , 41 , 42 , 46 , and 62 with concomitant extrusion of ethylene , in good yields .
	manualset3
172527	3	413403	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermolysis of 3 , 4-cis ring-fused 5-spirocyclopropane isoxazolidines 16 , 18-21 , 33 , 34 , 38a , and 61 , in the presence of a protic acid at 70-110 degrees C , yielded 3 , 4-cis ring-fused azetidin-2-ones 22-26 , 41 , 42 , 46 , and 62 with concomitant extrusion of ethylene , in good yields .
	manualset3
172528	4	413403	7	NULL	NULL	0	NULL	protic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermolysis of 3 , 4-cis ring-fused 5-spirocyclopropane isoxazolidines 16 , 18-21 , 33 , 34 , 38a , and 61 , in the presence of a protic acid at 70-110 degrees C , yielded 3 , 4-cis ring-fused azetidin-2-ones 22-26 , 41 , 42 , 46 , and 62 with concomitant extrusion of ethylene , in good yields .
	manualset3
172529	5	413403	7	NULL	NULL	0	NULL	70-110 degrees C	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermolysis of 3 , 4-cis ring-fused 5-spirocyclopropane isoxazolidines 16 , 18-21 , 33 , 34 , 38a , and 61 , in the presence of a protic acid at 70-110 degrees C , yielded 3 , 4-cis ring-fused azetidin-2-ones 22-26 , 41 , 42 , 46 , and 62 with concomitant extrusion of ethylene , in good yields .
	manualset3
172530	6	413403	7	NULL	NULL	0	NULL	3 , 4-cis ring-fused azetidin-2-ones 22-26 , 41 , 42 , 46 , and 62	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermolysis of 3 , 4-cis ring-fused 5-spirocyclopropane isoxazolidines 16 , 18-21 , 33 , 34 , 38a , and 61 , in the presence of a protic acid at 70-110 degrees C , yielded 3 , 4-cis ring-fused azetidin-2-ones 22-26 , 41 , 42 , 46 , and 62 with concomitant extrusion of ethylene , in good yields .
	manualset3
172531	7	413403	7	NULL	NULL	0	NULL	concomitant extrusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermolysis of 3 , 4-cis ring-fused 5-spirocyclopropane isoxazolidines 16 , 18-21 , 33 , 34 , 38a , and 61 , in the presence of a protic acid at 70-110 degrees C , yielded 3 , 4-cis ring-fused azetidin-2-ones 22-26 , 41 , 42 , 46 , and 62 with concomitant extrusion of ethylene , in good yields .
	manualset3
172532	8	413403	7	NULL	NULL	0	NULL	ethylene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermolysis of 3 , 4-cis ring-fused 5-spirocyclopropane isoxazolidines 16 , 18-21 , 33 , 34 , 38a , and 61 , in the presence of a protic acid at 70-110 degrees C , yielded 3 , 4-cis ring-fused azetidin-2-ones 22-26 , 41 , 42 , 46 , and 62 with concomitant extrusion of ethylene , in good yields .
	manualset3
172533	9	413403	7	NULL	NULL	0	NULL	good yields	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermolysis of 3 , 4-cis ring-fused 5-spirocyclopropane isoxazolidines 16 , 18-21 , 33 , 34 , 38a , and 61 , in the presence of a protic acid at 70-110 degrees C , yielded 3 , 4-cis ring-fused azetidin-2-ones 22-26 , 41 , 42 , 46 , and 62 with concomitant extrusion of ethylene , in good yields .
	manualset3
172534	1	413404	7	NULL	NULL	0	NULL	Thermus aquaticus MutS protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermus aquaticus MutS protein is a DNA mismatch repair protein that recognizes and binds to heteroduplex DNAs containing mispaired or unpaired bases .
	manualset3
172535	2	413404	7	NULL	NULL	0	NULL	DNA mismatch repair protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermus aquaticus MutS protein is a DNA mismatch repair protein that recognizes and binds to heteroduplex DNAs containing mispaired or unpaired bases .
	manualset3
172536	3	413404	7	NULL	NULL	0	NULL	heteroduplex DNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermus aquaticus MutS protein is a DNA mismatch repair protein that recognizes and binds to heteroduplex DNAs containing mispaired or unpaired bases .
	manualset3
172537	4	413404	7	NULL	NULL	0	NULL	mispaired bases	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermus aquaticus MutS protein is a DNA mismatch repair protein that recognizes and binds to heteroduplex DNAs containing mispaired or unpaired bases .
	manualset3
172538	5	413404	7	NULL	NULL	0	NULL	unpaired bases	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermus aquaticus MutS protein is a DNA mismatch repair protein that recognizes and binds to heteroduplex DNAs containing mispaired or unpaired bases .
	manualset3
172539	1	413405	7	NULL	NULL	0	NULL	terahertz Raman spectra	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These , along with the terahertz Raman spectra , show no evidence of the effects observed in amide systems , but display trends consistent with the presence of an equilibrium between the linear and cyclic dimer structures at all temperatures and moderate-to-high mole fractions in aqueous solution .
	manualset3
172540	2	413405	7	NULL	NULL	NULL	NULL	 evidence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These , along with the terahertz Raman spectra , show no evidence of the effects observed in amide systems , but display trends consistent with the presence of an equilibrium between the linear and cyclic dimer structures at all temperatures and moderate-to-high mole fractions in aqueous solution .
	manualset3
172541	3	413405	7	NULL	NULL	0	NULL	 effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These , along with the terahertz Raman spectra , show no evidence of the effects observed in amide systems , but display trends consistent with the presence of an equilibrium between the linear and cyclic dimer structures at all temperatures and moderate-to-high mole fractions in aqueous solution .
	manualset3
172542	4	413405	7	NULL	NULL	0	NULL	amide systems	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These , along with the terahertz Raman spectra , show no evidence of the effects observed in amide systems , but display trends consistent with the presence of an equilibrium between the linear and cyclic dimer structures at all temperatures and moderate-to-high mole fractions in aqueous solution .
	manualset3
172543	5	413405	7	NULL	NULL	0	NULL	 display	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These , along with the terahertz Raman spectra , show no evidence of the effects observed in amide systems , but display trends consistent with the presence of an equilibrium between the linear and cyclic dimer structures at all temperatures and moderate-to-high mole fractions in aqueous solution .
	manualset3
172544	6	413405	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These , along with the terahertz Raman spectra , show no evidence of the effects observed in amide systems , but display trends consistent with the presence of an equilibrium between the linear and cyclic dimer structures at all temperatures and moderate-to-high mole fractions in aqueous solution .
	manualset3
172545	7	413405	7	NULL	NULL	0	NULL	equilibrium	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These , along with the terahertz Raman spectra , show no evidence of the effects observed in amide systems , but display trends consistent with the presence of an equilibrium between the linear and cyclic dimer structures at all temperatures and moderate-to-high mole fractions in aqueous solution .
	manualset3
172546	8	413405	7	NULL	NULL	0	NULL	linear structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These , along with the terahertz Raman spectra , show no evidence of the effects observed in amide systems , but display trends consistent with the presence of an equilibrium between the linear and cyclic dimer structures at all temperatures and moderate-to-high mole fractions in aqueous solution .
	manualset3
172547	9	413405	7	NULL	NULL	0	NULL	cyclic dimer structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These , along with the terahertz Raman spectra , show no evidence of the effects observed in amide systems , but display trends consistent with the presence of an equilibrium between the linear and cyclic dimer structures at all temperatures and moderate-to-high mole fractions in aqueous solution .
	manualset3
172548	10	413405	7	NULL	NULL	0	NULL	temperatures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These , along with the terahertz Raman spectra , show no evidence of the effects observed in amide systems , but display trends consistent with the presence of an equilibrium between the linear and cyclic dimer structures at all temperatures and moderate-to-high mole fractions in aqueous solution .
	manualset3
172549	11	413405	7	NULL	NULL	0	NULL	moderate-to-high mole fractions	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These , along with the terahertz Raman spectra , show no evidence of the effects observed in amide systems , but display trends consistent with the presence of an equilibrium between the linear and cyclic dimer structures at all temperatures and moderate-to-high mole fractions in aqueous solution .
	manualset3
172550	12	413405	7	NULL	NULL	0	NULL	aqueous solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These , along with the terahertz Raman spectra , show no evidence of the effects observed in amide systems , but display trends consistent with the presence of an equilibrium between the linear and cyclic dimer structures at all temperatures and moderate-to-high mole fractions in aqueous solution .
	manualset3
172551	1	413406	7	NULL	NULL	0	NULL	3924A mitochondria	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These 3924A mitochondria fail to exhibit state 3 respiration when either pyruvate or citrate are supplied as respiratory fuels .
	manualset3
172552	2	413406	7	NULL	NULL	0	NULL	state 3 respiration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These 3924A mitochondria fail to exhibit state 3 respiration when either pyruvate or citrate are supplied as respiratory fuels .
	manualset3
172553	3	413406	7	NULL	NULL	0	NULL	 pyruvate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	These 3924A mitochondria fail to exhibit state 3 respiration when either pyruvate or citrate are supplied as respiratory fuels .
	manualset3
172554	4	413406	7	NULL	NULL	0	NULL	 citrate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	These 3924A mitochondria fail to exhibit state 3 respiration when either pyruvate or citrate are supplied as respiratory fuels .
	manualset3
172555	5	413406	7	NULL	NULL	0	NULL	respiratory fuels	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These 3924A mitochondria fail to exhibit state 3 respiration when either pyruvate or citrate are supplied as respiratory fuels .
	manualset3
172556	1	413407	7	NULL	NULL	0	NULL	 4-thiouridines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These 4-thiouridines serve as sites for conjugation of the cleavage reagent 5-iodoacetamido-1 , 10 - phenanthroline ( IOP ) .
	manualset3
172557	2	413407	7	NULL	NULL	0	NULL	sites	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These 4-thiouridines serve as sites for conjugation of the cleavage reagent 5-iodoacetamido-1 , 10 - phenanthroline ( IOP ) .
	manualset3
172558	3	413407	7	NULL	NULL	0	NULL	conjugation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These 4-thiouridines serve as sites for conjugation of the cleavage reagent 5-iodoacetamido-1 , 10 - phenanthroline ( IOP ) .
	manualset3
172559	4	413407	7	NULL	NULL	0	NULL	 cleavage reagent 5-iodoacetamido-1 , 10 - phenanthroline ( IOP )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These 4-thiouridines serve as sites for conjugation of the cleavage reagent 5-iodoacetamido-1 , 10 - phenanthroline ( IOP ) .
	manualset3
172560	1	413408	7	NULL	NULL	0	NULL	DNA lesions	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These DNA lesions represented direct DNA breaks .
	manualset3
172561	2	413408	7	NULL	NULL	0	NULL	direct DNA breaks	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These DNA lesions represented direct DNA breaks .
	manualset3
172562	1	413409	7	NULL	NULL	0	NULL	PCR-based typing methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These PCR-based typing methods , although they do not permit determination of the species of the isolates , are simple to perform and are suitable for clinical and ecological investigations of viridans group streptococci .
	manualset3
172563	2	413409	7	NULL	NULL	0	NULL	determination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These PCR-based typing methods , although they do not permit determination of the species of the isolates , are simple to perform and are suitable for clinical and ecological investigations of viridans group streptococci .
	manualset3
172564	3	413409	7	NULL	NULL	0	NULL	species	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These PCR-based typing methods , although they do not permit determination of the species of the isolates , are simple to perform and are suitable for clinical and ecological investigations of viridans group streptococci .
	manualset3
172565	4	413409	7	NULL	NULL	0	NULL	 isolates	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These PCR-based typing methods , although they do not permit determination of the species of the isolates , are simple to perform and are suitable for clinical and ecological investigations of viridans group streptococci .
	manualset3
172566	5	413409	7	NULL	NULL	0	NULL	clinical investigation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These PCR-based typing methods , although they do not permit determination of the species of the isolates , are simple to perform and are suitable for clinical and ecological investigations of viridans group streptococci .
	manualset3
172567	6	413409	7	NULL	NULL	0	NULL	ecological investigations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These PCR-based typing methods , although they do not permit determination of the species of the isolates , are simple to perform and are suitable for clinical and ecological investigations of viridans group streptococci .
	manualset3
172568	7	413409	7	NULL	NULL	0	NULL	viridans group 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These PCR-based typing methods , although they do not permit determination of the species of the isolates , are simple to perform and are suitable for clinical and ecological investigations of viridans group streptococci .
	manualset3
172569	8	413409	7	NULL	NULL	0	NULL	 streptococci	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These PCR-based typing methods , although they do not permit determination of the species of the isolates , are simple to perform and are suitable for clinical and ecological investigations of viridans group streptococci .
	manualset3
172570	1	413410	7	NULL	NULL	0	NULL	PRC1-mediated modifications	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These PRC1-mediated modifications to the cytokinetic mechanism may be related to the specialization of the midbody in neural cells .
	manualset3
172571	2	413410	7	NULL	NULL	0	NULL	cytokinetic mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These PRC1-mediated modifications to the cytokinetic mechanism may be related to the specialization of the midbody in neural cells .
	manualset3
172572	3	413410	7	NULL	NULL	0	NULL	specialization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These PRC1-mediated modifications to the cytokinetic mechanism may be related to the specialization of the midbody in neural cells .
	manualset3
172573	4	413410	7	NULL	NULL	NULL	NULL	midbody	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These PRC1-mediated modifications to the cytokinetic mechanism may be related to the specialization of the midbody in neural cells .
	manualset3
172574	5	413410	7	NULL	NULL	0	NULL	neural cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These PRC1-mediated modifications to the cytokinetic mechanism may be related to the specialization of the midbody in neural cells .
	manualset3
172575	1	413411	7	NULL	NULL	0	NULL	RNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These RNAs act under various growth and stress conditions , suggesting that one important physiological role of regulatory RNA molecules in Gram-negative bacteria is to modulate the cell surface and/or to prevent accumulation of OMPs in the envelope .
	manualset3
172576	2	413411	7	NULL	NULL	NULL	NULL	growth conditions	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These RNAs act under various growth and stress conditions , suggesting that one important physiological role of regulatory RNA molecules in Gram-negative bacteria is to modulate the cell surface and/or to prevent accumulation of OMPs in the envelope .
	manualset3
172577	3	413411	7	NULL	NULL	NULL	NULL	stress conditions	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These RNAs act under various growth and stress conditions , suggesting that one important physiological role of regulatory RNA molecules in Gram-negative bacteria is to modulate the cell surface and/or to prevent accumulation of OMPs in the envelope .
	manualset3
172578	4	413411	7	NULL	NULL	0	NULL	 physiological role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These RNAs act under various growth and stress conditions , suggesting that one important physiological role of regulatory RNA molecules in Gram-negative bacteria is to modulate the cell surface and/or to prevent accumulation of OMPs in the envelope .
	manualset3
172579	5	413411	7	NULL	NULL	0	NULL	regulatory RNA molecules	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These RNAs act under various growth and stress conditions , suggesting that one important physiological role of regulatory RNA molecules in Gram-negative bacteria is to modulate the cell surface and/or to prevent accumulation of OMPs in the envelope .
	manualset3
172580	6	413411	7	NULL	NULL	0	NULL	Gram-negative bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These RNAs act under various growth and stress conditions , suggesting that one important physiological role of regulatory RNA molecules in Gram-negative bacteria is to modulate the cell surface and/or to prevent accumulation of OMPs in the envelope .
	manualset3
172581	7	413411	7	NULL	NULL	0	NULL	cell surface	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These RNAs act under various growth and stress conditions , suggesting that one important physiological role of regulatory RNA molecules in Gram-negative bacteria is to modulate the cell surface and/or to prevent accumulation of OMPs in the envelope .
	manualset3
172582	8	413411	7	NULL	NULL	0	NULL	accumulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These RNAs act under various growth and stress conditions , suggesting that one important physiological role of regulatory RNA molecules in Gram-negative bacteria is to modulate the cell surface and/or to prevent accumulation of OMPs in the envelope .
	manualset3
172583	9	413411	7	NULL	NULL	0	NULL	 OMPs	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These RNAs act under various growth and stress conditions , suggesting that one important physiological role of regulatory RNA molecules in Gram-negative bacteria is to modulate the cell surface and/or to prevent accumulation of OMPs in the envelope .
	manualset3
172584	10	413411	7	NULL	NULL	0	NULL	envelope	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These RNAs act under various growth and stress conditions , suggesting that one important physiological role of regulatory RNA molecules in Gram-negative bacteria is to modulate the cell surface and/or to prevent accumulation of OMPs in the envelope .
	manualset3
172585	1	413412	7	NULL	NULL	0	NULL	RNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These RNAs are rapidly degraded , as are other mRNAs , after fertilization and prior to the second cleavage .
	manualset3
172586	2	413412	7	NULL	NULL	0	NULL	mRNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These RNAs are rapidly degraded , as are other mRNAs , after fertilization and prior to the second cleavage .
	manualset3
172587	3	413412	7	NULL	NULL	0	NULL	fertilization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These RNAs are rapidly degraded , as are other mRNAs , after fertilization and prior to the second cleavage .
	manualset3
172588	4	413412	7	NULL	NULL	0	NULL	second cleavage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These RNAs are rapidly degraded , as are other mRNAs , after fertilization and prior to the second cleavage .
	manualset3
172589	1	413413	7	NULL	NULL	0	NULL	SNPs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These SNPs are located within 4 kb of the 5 ' UTR of GPCPD1 , glycerophosphocholine phosphodiesterase GDE1 homolog ( Saccharomyces cerevisiae ) , which in humans , is more highly expressed in occipital cortex compared with the remainder of cortex than 99.9 % of genes genome-wide .
	manualset3
172590	2	413413	7	NULL	NULL	0	NULL	4 kb	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These SNPs are located within 4 kb of the 5 ' UTR of GPCPD1 , glycerophosphocholine phosphodiesterase GDE1 homolog ( Saccharomyces cerevisiae ) , which in humans , is more highly expressed in occipital cortex compared with the remainder of cortex than 99.9 % of genes genome-wide .
	manualset3
172591	3	413413	7	NULL	NULL	0	NULL	 5 ' UTR	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These SNPs are located within 4 kb of the 5 ' UTR of GPCPD1 , glycerophosphocholine phosphodiesterase GDE1 homolog ( Saccharomyces cerevisiae ) , which in humans , is more highly expressed in occipital cortex compared with the remainder of cortex than 99.9 % of genes genome-wide .
	manualset3
172592	4	413413	7	NULL	NULL	NULL	NULL	GPCPD1	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These SNPs are located within 4 kb of the 5 ' UTR of GPCPD1 , glycerophosphocholine phosphodiesterase GDE1 homolog ( Saccharomyces cerevisiae ) , which in humans , is more highly expressed in occipital cortex compared with the remainder of cortex than 99.9 % of genes genome-wide .
	manualset3
172593	5	413413	7	NULL	NULL	0	NULL	glycerophosphocholine phosphodiesterase GDE1 homolog 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These SNPs are located within 4 kb of the 5 ' UTR of GPCPD1 , glycerophosphocholine phosphodiesterase GDE1 homolog ( Saccharomyces cerevisiae ) , which in humans , is more highly expressed in occipital cortex compared with the remainder of cortex than 99.9 % of genes genome-wide .
	manualset3
172594	6	413413	7	NULL	NULL	0	NULL	Saccharomyces cerevisiae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These SNPs are located within 4 kb of the 5 ' UTR of GPCPD1 , glycerophosphocholine phosphodiesterase GDE1 homolog ( Saccharomyces cerevisiae ) , which in humans , is more highly expressed in occipital cortex compared with the remainder of cortex than 99.9 % of genes genome-wide .
	manualset3
172595	7	413413	7	NULL	NULL	0	NULL	humans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These SNPs are located within 4 kb of the 5 ' UTR of GPCPD1 , glycerophosphocholine phosphodiesterase GDE1 homolog ( Saccharomyces cerevisiae ) , which in humans , is more highly expressed in occipital cortex compared with the remainder of cortex than 99.9 % of genes genome-wide .
	manualset3
172596	8	413413	7	NULL	NULL	0	NULL	occipital cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These SNPs are located within 4 kb of the 5 ' UTR of GPCPD1 , glycerophosphocholine phosphodiesterase GDE1 homolog ( Saccharomyces cerevisiae ) , which in humans , is more highly expressed in occipital cortex compared with the remainder of cortex than 99.9 % of genes genome-wide .
	manualset3
172597	9	413413	7	NULL	NULL	0	NULL	remainder	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These SNPs are located within 4 kb of the 5 ' UTR of GPCPD1 , glycerophosphocholine phosphodiesterase GDE1 homolog ( Saccharomyces cerevisiae ) , which in humans , is more highly expressed in occipital cortex compared with the remainder of cortex than 99.9 % of genes genome-wide .
	manualset3
172598	10	413413	7	NULL	NULL	0	NULL	cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These SNPs are located within 4 kb of the 5 ' UTR of GPCPD1 , glycerophosphocholine phosphodiesterase GDE1 homolog ( Saccharomyces cerevisiae ) , which in humans , is more highly expressed in occipital cortex compared with the remainder of cortex than 99.9 % of genes genome-wide .
	manualset3
172599	11	413413	7	NULL	NULL	0	NULL	 99.9 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These SNPs are located within 4 kb of the 5 ' UTR of GPCPD1 , glycerophosphocholine phosphodiesterase GDE1 homolog ( Saccharomyces cerevisiae ) , which in humans , is more highly expressed in occipital cortex compared with the remainder of cortex than 99.9 % of genes genome-wide .
	manualset3
172600	12	413413	7	NULL	NULL	0	NULL	genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	These SNPs are located within 4 kb of the 5 ' UTR of GPCPD1 , glycerophosphocholine phosphodiesterase GDE1 homolog ( Saccharomyces cerevisiae ) , which in humans , is more highly expressed in occipital cortex compared with the remainder of cortex than 99.9 % of genes genome-wide .
	manualset3
172601	1	413414	7	NULL	NULL	0	NULL	TAAs	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These TAAs may play an important role in the antitumor surveillance mechanism by the host immune system .
	manualset3
172602	2	413414	7	NULL	NULL	0	NULL	 role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These TAAs may play an important role in the antitumor surveillance mechanism by the host immune system .
	manualset3
172603	3	413414	7	NULL	NULL	0	NULL	antitumor surveillance mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These TAAs may play an important role in the antitumor surveillance mechanism by the host immune system .
	manualset3
172604	4	413414	7	NULL	NULL	NULL	NULL	host immune system	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These TAAs may play an important role in the antitumor surveillance mechanism by the host immune system .
	manualset3
172605	1	413415	7	NULL	NULL	0	NULL	Th1-dominated responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These Th1-dominated responses were CD4 , CD8 , CD86 dependent , and were closely paralleled by strong virus-driven IL-10 and CCL5 production .
	manualset3
172606	2	413415	7	NULL	NULL	0	NULL	CD4 dependent	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These Th1-dominated responses were CD4 , CD8 , CD86 dependent , and were closely paralleled by strong virus-driven IL-10 and CCL5 production .
	manualset3
172607	3	413415	7	NULL	NULL	0	NULL	 CD8 dependent	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These Th1-dominated responses were CD4 , CD8 , CD86 dependent , and were closely paralleled by strong virus-driven IL-10 and CCL5 production .
	manualset3
172608	4	413415	7	NULL	NULL	0	NULL	CD86 dependent	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These Th1-dominated responses were CD4 , CD8 , CD86 dependent , and were closely paralleled by strong virus-driven IL-10 and CCL5 production .
	manualset3
172609	5	413415	7	NULL	NULL	0	NULL	 virus-driven IL-10 production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These Th1-dominated responses were CD4 , CD8 , CD86 dependent , and were closely paralleled by strong virus-driven IL-10 and CCL5 production .
	manualset3
172610	6	413415	7	NULL	NULL	0	NULL	CCL5 production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These Th1-dominated responses were CD4 , CD8 , CD86 dependent , and were closely paralleled by strong virus-driven IL-10 and CCL5 production .
	manualset3
172611	1	413416	7	NULL	NULL	0	NULL	Acute fatty liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute fatty liver of pregnancy .
	manualset3
172612	2	413416	7	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute fatty liver of pregnancy .
	manualset3
172613	1	413417	7	NULL	NULL	0	NULL	ZAP-70-deficient mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These ZAP-70-deficient mice that received an IT transplant had a significantly increased prothymocyte niche compared with their untreated counterparts ; this phenotype was associated with the generation of a medulla .
	manualset3
172614	2	413417	7	NULL	NULL	0	NULL	IT transplant	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These ZAP-70-deficient mice that received an IT transplant had a significantly increased prothymocyte niche compared with their untreated counterparts ; this phenotype was associated with the generation of a medulla .
	manualset3
172615	3	413417	7	NULL	NULL	0	NULL	prothymocyte	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These ZAP-70-deficient mice that received an IT transplant had a significantly increased prothymocyte niche compared with their untreated counterparts ; this phenotype was associated with the generation of a medulla .
	manualset3
172616	4	413417	7	NULL	NULL	NULL	NULL	untreated counterparts	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These ZAP-70-deficient mice that received an IT transplant had a significantly increased prothymocyte niche compared with their untreated counterparts ; this phenotype was associated with the generation of a medulla .
	manualset3
172617	5	413417	7	NULL	NULL	0	NULL	phenotype	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These ZAP-70-deficient mice that received an IT transplant had a significantly increased prothymocyte niche compared with their untreated counterparts ; this phenotype was associated with the generation of a medulla .
	manualset3
172618	6	413417	7	NULL	NULL	0	NULL	generation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These ZAP-70-deficient mice that received an IT transplant had a significantly increased prothymocyte niche compared with their untreated counterparts ; this phenotype was associated with the generation of a medulla .
	manualset3
172619	7	413417	7	NULL	NULL	0	NULL	medulla	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These ZAP-70-deficient mice that received an IT transplant had a significantly increased prothymocyte niche compared with their untreated counterparts ; this phenotype was associated with the generation of a medulla .
	manualset3
172620	1	413418	7	NULL	NULL	0	NULL	action-orientated systems	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These action-orientated systems , described in neuropsychological terms , give rise to negative emotions that include fear , anger and panic , and positive emotions that include comfort , vitality , euphoria and playfulness .
	manualset3
172625	2	413418	7	NULL	NULL	0	NULL	neuropsychological terms	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These action-orientated systems , described in neuropsychological terms , give rise to negative emotions that include fear , anger and panic , and positive emotions that include comfort , vitality , euphoria and playfulness .
	manualset3
172627	3	413418	7	NULL	NULL	0	NULL	negative emotions	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These action-orientated systems , described in neuropsychological terms , give rise to negative emotions that include fear , anger and panic , and positive emotions that include comfort , vitality , euphoria and playfulness .
	manualset3
172628	4	413418	7	NULL	NULL	0	NULL	 fear	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These action-orientated systems , described in neuropsychological terms , give rise to negative emotions that include fear , anger and panic , and positive emotions that include comfort , vitality , euphoria and playfulness .
	manualset3
172629	5	413418	7	NULL	NULL	0	NULL	anger 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These action-orientated systems , described in neuropsychological terms , give rise to negative emotions that include fear , anger and panic , and positive emotions that include comfort , vitality , euphoria and playfulness .
	manualset3
172630	6	413418	7	NULL	NULL	0	NULL	panic	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These action-orientated systems , described in neuropsychological terms , give rise to negative emotions that include fear , anger and panic , and positive emotions that include comfort , vitality , euphoria and playfulness .
	manualset3
172631	7	413418	7	NULL	NULL	0	NULL	positive emotions	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These action-orientated systems , described in neuropsychological terms , give rise to negative emotions that include fear , anger and panic , and positive emotions that include comfort , vitality , euphoria and playfulness .
	manualset3
172632	8	413418	7	NULL	NULL	0	NULL	 comfort	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These action-orientated systems , described in neuropsychological terms , give rise to negative emotions that include fear , anger and panic , and positive emotions that include comfort , vitality , euphoria and playfulness .
	manualset3
172633	9	413418	7	NULL	NULL	0	NULL	vitality	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These action-orientated systems , described in neuropsychological terms , give rise to negative emotions that include fear , anger and panic , and positive emotions that include comfort , vitality , euphoria and playfulness .
	manualset3
172634	10	413418	7	NULL	NULL	0	NULL	euphoria 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These action-orientated systems , described in neuropsychological terms , give rise to negative emotions that include fear , anger and panic , and positive emotions that include comfort , vitality , euphoria and playfulness .
	manualset3
172635	11	413418	7	NULL	NULL	0	NULL	playfulness	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These action-orientated systems , described in neuropsychological terms , give rise to negative emotions that include fear , anger and panic , and positive emotions that include comfort , vitality , euphoria and playfulness .
	manualset3
172636	1	413419	7	NULL	NULL	0	NULL	activities 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These activities can lead to the exhausting of the reservoir of future cases by preventing reactivation .
	manualset3
172637	2	413419	7	NULL	NULL	0	NULL	reservoir	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These activities can lead to the exhausting of the reservoir of future cases by preventing reactivation .
	manualset3
172638	3	413419	7	NULL	NULL	NULL	NULL	future cases	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These activities can lead to the exhausting of the reservoir of future cases by preventing reactivation .
	manualset3
172639	4	413419	7	NULL	NULL	0	NULL	reactivation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These activities can lead to the exhausting of the reservoir of future cases by preventing reactivation .
	manualset3
172640	1	413420	7	NULL	NULL	0	NULL	activities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These activities have resulted in intensified co-operation between the USA and the EU .
	manualset3
172641	2	413420	7	NULL	NULL	0	NULL	intensified co-operation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These activities have resulted in intensified co-operation between the USA and the EU .
	manualset3
172642	3	413420	7	NULL	NULL	0	NULL	USA	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	These activities have resulted in intensified co-operation between the USA and the EU .
	manualset3
172643	4	413420	7	NULL	NULL	0	NULL	EU	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	These activities have resulted in intensified co-operation between the USA and the EU .
	manualset3
172644	1	413421	7	NULL	NULL	0	NULL	adaptive changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These adaptive changes are another factor potentially limiting the strength of the relationship between MRI measures of pathology and clinical measures of disability .
	manualset3
172645	2	413421	7	NULL	NULL	0	NULL	factor	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These adaptive changes are another factor potentially limiting the strength of the relationship between MRI measures of pathology and clinical measures of disability .
	manualset3
172646	3	413421	7	NULL	NULL	0	NULL	strength	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These adaptive changes are another factor potentially limiting the strength of the relationship between MRI measures of pathology and clinical measures of disability .
	manualset3
172647	4	413421	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These adaptive changes are another factor potentially limiting the strength of the relationship between MRI measures of pathology and clinical measures of disability .
	manualset3
172648	5	413421	7	NULL	NULL	0	NULL	MRI measures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These adaptive changes are another factor potentially limiting the strength of the relationship between MRI measures of pathology and clinical measures of disability .
	manualset3
172649	6	413421	7	NULL	NULL	0	NULL	pathology 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These adaptive changes are another factor potentially limiting the strength of the relationship between MRI measures of pathology and clinical measures of disability .
	manualset3
172650	7	413421	7	NULL	NULL	0	NULL	clinical measures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These adaptive changes are another factor potentially limiting the strength of the relationship between MRI measures of pathology and clinical measures of disability .
	manualset3
172651	8	413421	7	NULL	NULL	0	NULL	disability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These adaptive changes are another factor potentially limiting the strength of the relationship between MRI measures of pathology and clinical measures of disability .
	manualset3
172652	1	413422	7	NULL	NULL	0	NULL	 alterations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These alterations are more pronounced and occur sooner in prosthesis with parts ( rotation ball or cup . )
	manualset3
172653	2	413422	7	NULL	NULL	NULL	NULL	prosthesis with parts	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These alterations are more pronounced and occur sooner in prosthesis with parts ( rotation ball or cup . )
	manualset3
172654	3	413422	7	NULL	NULL	NULL	NULL	 rotation ball or cup	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These alterations are more pronounced and occur sooner in prosthesis with parts ( rotation ball or cup . )
	manualset3
172655	1	413423	7	NULL	NULL	0	NULL	 amounts 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These amounts of this antibody protect leukopenic rabbits against the lethality of the slow onset bacteremic model of Pseudomonas conjunctivitis .
	manualset3
172656	2	413423	7	NULL	NULL	0	NULL	antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These amounts of this antibody protect leukopenic rabbits against the lethality of the slow onset bacteremic model of Pseudomonas conjunctivitis .
	manualset3
172657	3	413423	7	NULL	NULL	0	NULL	leukopenic rabbits	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These amounts of this antibody protect leukopenic rabbits against the lethality of the slow onset bacteremic model of Pseudomonas conjunctivitis .
	manualset3
172658	4	413423	7	NULL	NULL	0	NULL	lethality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These amounts of this antibody protect leukopenic rabbits against the lethality of the slow onset bacteremic model of Pseudomonas conjunctivitis .
	manualset3
172659	5	413423	7	NULL	NULL	0	NULL	slow onset bacteremic model	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These amounts of this antibody protect leukopenic rabbits against the lethality of the slow onset bacteremic model of Pseudomonas conjunctivitis .
	manualset3
172660	6	413423	7	NULL	NULL	0	NULL	Pseudomonas conjunctivitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These amounts of this antibody protect leukopenic rabbits against the lethality of the slow onset bacteremic model of Pseudomonas conjunctivitis .
	manualset3
172661	1	413424	7	NULL	NULL	0	NULL	analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These analyses suggest a strict requirement for a specific proline residue adjacent to the inhibitor reactive site and give additional insights for future phage display application .
	manualset3
172662	2	413424	7	NULL	NULL	0	NULL	strict requirement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These analyses suggest a strict requirement for a specific proline residue adjacent to the inhibitor reactive site and give additional insights for future phage display application .
	manualset3
172663	3	413424	7	NULL	NULL	0	NULL	proline residue	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These analyses suggest a strict requirement for a specific proline residue adjacent to the inhibitor reactive site and give additional insights for future phage display application .
	manualset3
172664	4	413424	7	NULL	NULL	0	NULL	inhibitor reactive site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These analyses suggest a strict requirement for a specific proline residue adjacent to the inhibitor reactive site and give additional insights for future phage display application .
	manualset3
172665	5	413424	7	NULL	NULL	0	NULL	 insights	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These analyses suggest a strict requirement for a specific proline residue adjacent to the inhibitor reactive site and give additional insights for future phage display application .
	manualset3
172666	6	413424	7	NULL	NULL	NULL	NULL	phage display application	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These analyses suggest a strict requirement for a specific proline residue adjacent to the inhibitor reactive site and give additional insights for future phage display application .
	manualset3
172667	1	413425	7	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These and other differences suggest that endosperm slices are freely permeable to sugars .
	manualset3
172668	2	413425	7	NULL	NULL	0	NULL	endosperm slices	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These and other differences suggest that endosperm slices are freely permeable to sugars .
	manualset3
172669	3	413425	7	NULL	NULL	0	NULL	permeable 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These and other differences suggest that endosperm slices are freely permeable to sugars .
	manualset3
172670	4	413425	7	NULL	NULL	0	NULL	 sugars	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These and other differences suggest that endosperm slices are freely permeable to sugars .
	manualset3
172671	1	413426	7	NULL	NULL	0	NULL	constituents	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These and other useful constituents e.g. protein C activator and platelet aggregating agents are discussed .
	manualset3
172672	2	413426	7	NULL	NULL	NULL	NULL	protein C activator	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These and other useful constituents e.g. protein C activator and platelet aggregating agents are discussed .
	manualset3
172673	3	413426	7	NULL	NULL	0	NULL	platelet aggregating agents	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These and other useful constituents e.g. protein C activator and platelet aggregating agents are discussed .
	manualset3
172674	1	413427	7	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These animals may serve as an in vivo system for culturing HCV and addressing pathophysiological and therapeutic issues of HCV infection .
	manualset3
172675	2	413427	7	NULL	NULL	0	NULL	in vivo system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These animals may serve as an in vivo system for culturing HCV and addressing pathophysiological and therapeutic issues of HCV infection .
	manualset3
172676	3	413427	7	NULL	NULL	NULL	NULL	 culturing HCV	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These animals may serve as an in vivo system for culturing HCV and addressing pathophysiological and therapeutic issues of HCV infection .
	manualset3
172677	4	413427	7	NULL	NULL	0	NULL	pathophysiological issues	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These animals may serve as an in vivo system for culturing HCV and addressing pathophysiological and therapeutic issues of HCV infection .
	manualset3
172678	5	413427	7	NULL	NULL	0	NULL	therapeutic issues	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These animals may serve as an in vivo system for culturing HCV and addressing pathophysiological and therapeutic issues of HCV infection .
	manualset3
172679	6	413427	7	NULL	NULL	0	NULL	HCV infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These animals may serve as an in vivo system for culturing HCV and addressing pathophysiological and therapeutic issues of HCV infection .
	manualset3
172680	1	413428	7	NULL	NULL	0	NULL	animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These animals present an accelerated time course of hypertension and a reduced life-span .
	manualset3
172681	2	413428	7	NULL	NULL	0	NULL	accelerated time course	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	These animals present an accelerated time course of hypertension and a reduced life-span .
	manualset3
172682	3	413428	7	NULL	NULL	0	NULL	hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These animals present an accelerated time course of hypertension and a reduced life-span .
	manualset3
172683	4	413428	7	NULL	NULL	0	NULL	 reduced life-span	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These animals present an accelerated time course of hypertension and a reduced life-span .
	manualset3
172684	1	413429	7	NULL	NULL	0	NULL	animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These animals show no cerebral lesions that are reputed characteristics of human dementia , such as tangles or amyloid plaques .
	manualset3
172685	2	413429	7	NULL	NULL	0	NULL	 cerebral lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These animals show no cerebral lesions that are reputed characteristics of human dementia , such as tangles or amyloid plaques .
	manualset3
172686	3	413429	7	NULL	NULL	0	NULL	human dementia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These animals show no cerebral lesions that are reputed characteristics of human dementia , such as tangles or amyloid plaques .
	manualset3
172687	4	413429	7	NULL	NULL	0	NULL	tangles	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These animals show no cerebral lesions that are reputed characteristics of human dementia , such as tangles or amyloid plaques .
	manualset3
172688	5	413429	7	NULL	NULL	0	NULL	amyloid plaques	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These animals show no cerebral lesions that are reputed characteristics of human dementia , such as tangles or amyloid plaques .
	manualset3
172689	1	413430	7	NULL	NULL	0	NULL	anion-dependent natures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These anion-dependent natures of the chromoionophore allowed us to detect acetate and phosphate ions easily .
	manualset3
172690	2	413430	7	NULL	NULL	0	NULL	 chromoionophore 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These anion-dependent natures of the chromoionophore allowed us to detect acetate and phosphate ions easily .
	manualset3
172691	3	413430	7	NULL	NULL	0	NULL	acetate ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	These anion-dependent natures of the chromoionophore allowed us to detect acetate and phosphate ions easily .
	manualset3
172692	4	413430	7	NULL	NULL	0	NULL	phosphate ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	These anion-dependent natures of the chromoionophore allowed us to detect acetate and phosphate ions easily .
	manualset3
172707	1	413431	7	NULL	NULL	0	NULL	antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These antibodies ( termed anti-Ub ) had no effect on the sodium-independent uptake of these substances or their calcium-dependent efflux .
	manualset3
172708	2	413431	7	NULL	NULL	0	NULL	anti-Ub	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These antibodies ( termed anti-Ub ) had no effect on the sodium-independent uptake of these substances or their calcium-dependent efflux .
	manualset3
172709	3	413431	7	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These antibodies ( termed anti-Ub ) had no effect on the sodium-independent uptake of these substances or their calcium-dependent efflux .
	manualset3
172710	4	413431	7	NULL	NULL	0	NULL	sodium-independent uptake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These antibodies ( termed anti-Ub ) had no effect on the sodium-independent uptake of these substances or their calcium-dependent efflux .
	manualset3
172711	5	413431	7	NULL	NULL	0	NULL	substances	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These antibodies ( termed anti-Ub ) had no effect on the sodium-independent uptake of these substances or their calcium-dependent efflux .
	manualset3
172712	6	413431	7	NULL	NULL	0	NULL	calcium-dependent efflux 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These antibodies ( termed anti-Ub ) had no effect on the sodium-independent uptake of these substances or their calcium-dependent efflux .
	manualset3
172713	1	413432	7	NULL	NULL	0	NULL	 antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These antibodies and antigen detection methods may be useful to study pathological changes of mEH in various human diseases .
	manualset3
172714	2	413432	7	NULL	NULL	0	NULL	antigen detection methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These antibodies and antigen detection methods may be useful to study pathological changes of mEH in various human diseases .
	manualset3
172715	3	413432	7	NULL	NULL	NULL	NULL	pathological changes	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These antibodies and antigen detection methods may be useful to study pathological changes of mEH in various human diseases .
	manualset3
172716	4	413432	7	NULL	NULL	0	NULL	 mEH	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These antibodies and antigen detection methods may be useful to study pathological changes of mEH in various human diseases .
	manualset3
172717	5	413432	7	NULL	NULL	0	NULL	human diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These antibodies and antigen detection methods may be useful to study pathological changes of mEH in various human diseases .
	manualset3
172718	1	413433	7	NULL	NULL	0	NULL	first examples	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These are the first examples linking the PHD domain to E3 activity , but the recent discovery of PHD-dependent E3 activity in the cellular kinase MEKK1 and the close structural relation of PHD domains to RING fingers hint that many other PHD proteins might share this activity .
	manualset3
172719	2	413433	7	NULL	NULL	0	NULL	 PHD domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These are the first examples linking the PHD domain to E3 activity , but the recent discovery of PHD-dependent E3 activity in the cellular kinase MEKK1 and the close structural relation of PHD domains to RING fingers hint that many other PHD proteins might share this activity .
	manualset3
172720	3	413433	7	NULL	NULL	0	NULL	E3 activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These are the first examples linking the PHD domain to E3 activity , but the recent discovery of PHD-dependent E3 activity in the cellular kinase MEKK1 and the close structural relation of PHD domains to RING fingers hint that many other PHD proteins might share this activity .
	manualset3
172721	4	413433	7	NULL	NULL	0	NULL	 recent discovery 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These are the first examples linking the PHD domain to E3 activity , but the recent discovery of PHD-dependent E3 activity in the cellular kinase MEKK1 and the close structural relation of PHD domains to RING fingers hint that many other PHD proteins might share this activity .
	manualset3
172722	5	413433	7	NULL	NULL	0	NULL	PHD-dependent E3 activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These are the first examples linking the PHD domain to E3 activity , but the recent discovery of PHD-dependent E3 activity in the cellular kinase MEKK1 and the close structural relation of PHD domains to RING fingers hint that many other PHD proteins might share this activity .
	manualset3
172723	6	413433	7	NULL	NULL	0	NULL	cellular kinase MEKK1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These are the first examples linking the PHD domain to E3 activity , but the recent discovery of PHD-dependent E3 activity in the cellular kinase MEKK1 and the close structural relation of PHD domains to RING fingers hint that many other PHD proteins might share this activity .
	manualset3
172724	7	413433	7	NULL	NULL	0	NULL	structural relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These are the first examples linking the PHD domain to E3 activity , but the recent discovery of PHD-dependent E3 activity in the cellular kinase MEKK1 and the close structural relation of PHD domains to RING fingers hint that many other PHD proteins might share this activity .
	manualset3
172725	8	413433	7	NULL	NULL	0	NULL	PHD domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These are the first examples linking the PHD domain to E3 activity , but the recent discovery of PHD-dependent E3 activity in the cellular kinase MEKK1 and the close structural relation of PHD domains to RING fingers hint that many other PHD proteins might share this activity .
	manualset3
172726	9	413433	7	NULL	NULL	0	NULL	PHD proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These are the first examples linking the PHD domain to E3 activity , but the recent discovery of PHD-dependent E3 activity in the cellular kinase MEKK1 and the close structural relation of PHD domains to RING fingers hint that many other PHD proteins might share this activity .
	manualset3
172727	10	413433	7	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These are the first examples linking the PHD domain to E3 activity , but the recent discovery of PHD-dependent E3 activity in the cellular kinase MEKK1 and the close structural relation of PHD domains to RING fingers hint that many other PHD proteins might share this activity .
	manualset3
172728	11	413433	7	NULL	NULL	0	NULL	RING fingers	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These are the first examples linking the PHD domain to E3 activity , but the recent discovery of PHD-dependent E3 activity in the cellular kinase MEKK1 and the close structural relation of PHD domains to RING fingers hint that many other PHD proteins might share this activity .
	manualset3
172729	1	413434	7	NULL	NULL	0	NULL	artifacts	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These artifacts were not distributed uniformly , but were aligned at the frontotemporal base , close to the oropharynx .
	manualset3
172730	2	413434	7	NULL	NULL	0	NULL	frontotemporal base	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These artifacts were not distributed uniformly , but were aligned at the frontotemporal base , close to the oropharynx .
	manualset3
172731	4	413434	7	NULL	NULL	NULL	NULL	oropharynx	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These artifacts were not distributed uniformly , but were aligned at the frontotemporal base , close to the oropharynx .
	manualset3
172732	3	413434	7	NULL	NULL	0	NULL	close	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These artifacts were not distributed uniformly , but were aligned at the frontotemporal base , close to the oropharynx .
	manualset3
172733	1	413435	7	NULL	NULL	NULL	NULL	astrocytes	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These astrocytes form a layer in the LR that lines the pores of the lamina cribrosa and separates the connective septa from the axon bundles in the RR .
	manualset3
172734	2	413435	7	NULL	NULL	NULL	NULL	layer	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These astrocytes form a layer in the LR that lines the pores of the lamina cribrosa and separates the connective septa from the axon bundles in the RR .
	manualset3
172735	3	413435	7	NULL	NULL	NULL	NULL	 LR	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These astrocytes form a layer in the LR that lines the pores of the lamina cribrosa and separates the connective septa from the axon bundles in the RR .
	manualset3
172736	4	413435	7	NULL	NULL	NULL	NULL	pores	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These astrocytes form a layer in the LR that lines the pores of the lamina cribrosa and separates the connective septa from the axon bundles in the RR .
	manualset3
172737	5	413435	7	NULL	NULL	0	NULL	lamina cribrosa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These astrocytes form a layer in the LR that lines the pores of the lamina cribrosa and separates the connective septa from the axon bundles in the RR .
	manualset3
172738	6	413435	7	NULL	NULL	0	NULL	connective septa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These astrocytes form a layer in the LR that lines the pores of the lamina cribrosa and separates the connective septa from the axon bundles in the RR .
	manualset3
172739	7	413435	7	NULL	NULL	0	NULL	axon bundles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These astrocytes form a layer in the LR that lines the pores of the lamina cribrosa and separates the connective septa from the axon bundles in the RR .
	manualset3
172740	8	413435	7	NULL	NULL	0	NULL	RR	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These astrocytes form a layer in the LR that lines the pores of the lamina cribrosa and separates the connective septa from the axon bundles in the RR .
	manualset3
172741	1	413436	7	NULL	NULL	0	NULL	 beneficial effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These beneficial effects were associated with an increase in IL-10 secretion by immune cells of BBI-treated mice .
	manualset3
172742	2	413436	7	NULL	NULL	0	NULL	increase 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These beneficial effects were associated with an increase in IL-10 secretion by immune cells of BBI-treated mice .
	manualset3
172743	3	413436	7	NULL	NULL	0	NULL	IL-10 secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These beneficial effects were associated with an increase in IL-10 secretion by immune cells of BBI-treated mice .
	manualset3
172744	4	413436	7	NULL	NULL	0	NULL	immune cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These beneficial effects were associated with an increase in IL-10 secretion by immune cells of BBI-treated mice .
	manualset3
172745	5	413436	7	NULL	NULL	0	NULL	BBI-treated mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These beneficial effects were associated with an increase in IL-10 secretion by immune cells of BBI-treated mice .
	manualset3
172746	1	413437	7	NULL	NULL	0	NULL	interferon-beta ( IFN-beta ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute interferon-beta ( IFN-beta ) administration transiently activates the hypothalamic-pituitary-adrenal ( HPA ) axis , increases granulocytes , and reduces lymphocytes in peripheral blood .
	manualset3
172747	2	413437	7	NULL	NULL	0	NULL	Acute administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute interferon-beta ( IFN-beta ) administration transiently activates the hypothalamic-pituitary-adrenal ( HPA ) axis , increases granulocytes , and reduces lymphocytes in peripheral blood .
	manualset3
172748	3	413437	7	NULL	NULL	0	NULL	hypothalamic-pituitary-adrenal ( HPA ) axis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute interferon-beta ( IFN-beta ) administration transiently activates the hypothalamic-pituitary-adrenal ( HPA ) axis , increases granulocytes , and reduces lymphocytes in peripheral blood .
	manualset3
172749	4	413437	7	NULL	NULL	0	NULL	granulocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute interferon-beta ( IFN-beta ) administration transiently activates the hypothalamic-pituitary-adrenal ( HPA ) axis , increases granulocytes , and reduces lymphocytes in peripheral blood .
	manualset3
172750	5	413437	7	NULL	NULL	0	NULL	lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute interferon-beta ( IFN-beta ) administration transiently activates the hypothalamic-pituitary-adrenal ( HPA ) axis , increases granulocytes , and reduces lymphocytes in peripheral blood .
	manualset3
172751	6	413437	7	NULL	NULL	0	NULL	peripheral blood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute interferon-beta ( IFN-beta ) administration transiently activates the hypothalamic-pituitary-adrenal ( HPA ) axis , increases granulocytes , and reduces lymphocytes in peripheral blood .
	manualset3
172754	1	413438	7	NULL	NULL	0	NULL	biological effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These biological effects were obtained with levels of exogenous GATA-2 representing less than twofold increases over endogenous GATA-2 levels and were not observed in cells overexpressing GATA-1 / ER .
	manualset3
172755	2	413438	7	NULL	NULL	0	NULL	levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These biological effects were obtained with levels of exogenous GATA-2 representing less than twofold increases over endogenous GATA-2 levels and were not observed in cells overexpressing GATA-1 / ER .
	manualset3
172756	3	413438	7	NULL	NULL	0	NULL	exogenous GATA-2 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These biological effects were obtained with levels of exogenous GATA-2 representing less than twofold increases over endogenous GATA-2 levels and were not observed in cells overexpressing GATA-1 / ER .
	manualset3
172757	4	413438	7	NULL	NULL	0	NULL	 twofold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These biological effects were obtained with levels of exogenous GATA-2 representing less than twofold increases over endogenous GATA-2 levels and were not observed in cells overexpressing GATA-1 / ER .
	manualset3
172758	5	413438	7	NULL	NULL	0	NULL	endogenous GATA-2 levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These biological effects were obtained with levels of exogenous GATA-2 representing less than twofold increases over endogenous GATA-2 levels and were not observed in cells overexpressing GATA-1 / ER .
	manualset3
172759	6	413438	7	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These biological effects were obtained with levels of exogenous GATA-2 representing less than twofold increases over endogenous GATA-2 levels and were not observed in cells overexpressing GATA-1 / ER .
	manualset3
172760	7	413438	7	NULL	NULL	0	NULL	 GATA-1 / ER	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These biological effects were obtained with levels of exogenous GATA-2 representing less than twofold increases over endogenous GATA-2 levels and were not observed in cells overexpressing GATA-1 / ER .
	manualset3
172761	1	413439	7	NULL	NULL	0	NULL	biomechanical responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These biomechanical responses may be transmitted to the nucleus through cytoskeletal-linked signaling pathways .
	manualset3
172762	2	413439	7	NULL	NULL	0	NULL	nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These biomechanical responses may be transmitted to the nucleus through cytoskeletal-linked signaling pathways .
	manualset3
172763	3	413439	7	NULL	NULL	0	NULL	cytoskeletal-linked signaling pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These biomechanical responses may be transmitted to the nucleus through cytoskeletal-linked signaling pathways .
	manualset3
172764	1	413440	7	NULL	NULL	0	NULL	biospecific polymers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These biospecific polymers could presents sites of interaction with cell membrane receptors leading to modulation of cell biological activity .
	manualset3
172765	2	413440	7	NULL	NULL	0	NULL	 sites 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These biospecific polymers could presents sites of interaction with cell membrane receptors leading to modulation of cell biological activity .
	manualset3
172766	3	413440	7	NULL	NULL	0	NULL	interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These biospecific polymers could presents sites of interaction with cell membrane receptors leading to modulation of cell biological activity .
	manualset3
172767	4	413440	7	NULL	NULL	0	NULL	cell membrane receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These biospecific polymers could presents sites of interaction with cell membrane receptors leading to modulation of cell biological activity .
	manualset3
172768	5	413440	7	NULL	NULL	0	NULL	modulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These biospecific polymers could presents sites of interaction with cell membrane receptors leading to modulation of cell biological activity .
	manualset3
172769	6	413440	7	NULL	NULL	0	NULL	cell biological activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These biospecific polymers could presents sites of interaction with cell membrane receptors leading to modulation of cell biological activity .
	manualset3
172770	1	413441	7	NULL	NULL	0	NULL	biosurfactants	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These biosurfactants are composed of the disaccharide sophorose linked to a long-chain hydroxy fatty acid and have potential applications in the food , pharmaceutical , cosmetic and cleaning industries .
	manualset3
172771	2	413441	7	NULL	NULL	0	NULL	 disaccharide sophorose	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These biosurfactants are composed of the disaccharide sophorose linked to a long-chain hydroxy fatty acid and have potential applications in the food , pharmaceutical , cosmetic and cleaning industries .
	manualset3
172772	3	413441	7	NULL	NULL	0	NULL	long-chain hydroxy fatty acid	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These biosurfactants are composed of the disaccharide sophorose linked to a long-chain hydroxy fatty acid and have potential applications in the food , pharmaceutical , cosmetic and cleaning industries .
	manualset3
172773	4	413441	7	NULL	NULL	0	NULL	applications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These biosurfactants are composed of the disaccharide sophorose linked to a long-chain hydroxy fatty acid and have potential applications in the food , pharmaceutical , cosmetic and cleaning industries .
	manualset3
172774	5	413441	7	NULL	NULL	NULL	NULL	food industries	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These biosurfactants are composed of the disaccharide sophorose linked to a long-chain hydroxy fatty acid and have potential applications in the food , pharmaceutical , cosmetic and cleaning industries .
	manualset3
172775	6	413441	7	NULL	NULL	NULL	NULL	pharmaceutical industries	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These biosurfactants are composed of the disaccharide sophorose linked to a long-chain hydroxy fatty acid and have potential applications in the food , pharmaceutical , cosmetic and cleaning industries .
	manualset3
172776	7	413441	7	NULL	NULL	NULL	NULL	cosmetic industries	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These biosurfactants are composed of the disaccharide sophorose linked to a long-chain hydroxy fatty acid and have potential applications in the food , pharmaceutical , cosmetic and cleaning industries .
	manualset3
172777	8	413441	7	NULL	NULL	NULL	NULL	cleaning industries	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These biosurfactants are composed of the disaccharide sophorose linked to a long-chain hydroxy fatty acid and have potential applications in the food , pharmaceutical , cosmetic and cleaning industries .
	manualset3
172778	1	413442	7	NULL	NULL	0	NULL	bispecific antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These bispecific antibodies consist of a ` targeting ' domain , typically a fragment of a monoclonal antibody that binds to a tumor , linked to a ` triggering ' arm that is specific for a molecule capable of mediating a phagocytic or lytic response by macrophages , natural killer cells , T-cells or other effector cells .
	manualset3
172779	2	413442	7	NULL	NULL	0	NULL	` targeting ' domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These bispecific antibodies consist of a ` targeting ' domain , typically a fragment of a monoclonal antibody that binds to a tumor , linked to a ` triggering ' arm that is specific for a molecule capable of mediating a phagocytic or lytic response by macrophages , natural killer cells , T-cells or other effector cells .
	manualset3
172780	3	413442	7	NULL	NULL	0	NULL	fragment 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These bispecific antibodies consist of a ` targeting ' domain , typically a fragment of a monoclonal antibody that binds to a tumor , linked to a ` triggering ' arm that is specific for a molecule capable of mediating a phagocytic or lytic response by macrophages , natural killer cells , T-cells or other effector cells .
	manualset3
172781	4	413442	7	NULL	NULL	0	NULL	monoclonal antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These bispecific antibodies consist of a ` targeting ' domain , typically a fragment of a monoclonal antibody that binds to a tumor , linked to a ` triggering ' arm that is specific for a molecule capable of mediating a phagocytic or lytic response by macrophages , natural killer cells , T-cells or other effector cells .
	manualset3
172782	5	413442	7	NULL	NULL	0	NULL	 tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These bispecific antibodies consist of a ` targeting ' domain , typically a fragment of a monoclonal antibody that binds to a tumor , linked to a ` triggering ' arm that is specific for a molecule capable of mediating a phagocytic or lytic response by macrophages , natural killer cells , T-cells or other effector cells .
	manualset3
172783	6	413442	7	NULL	NULL	0	NULL	` triggering ' arm	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These bispecific antibodies consist of a ` targeting ' domain , typically a fragment of a monoclonal antibody that binds to a tumor , linked to a ` triggering ' arm that is specific for a molecule capable of mediating a phagocytic or lytic response by macrophages , natural killer cells , T-cells or other effector cells .
	manualset3
172784	7	413442	7	NULL	NULL	0	NULL	molecule 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	These bispecific antibodies consist of a ` targeting ' domain , typically a fragment of a monoclonal antibody that binds to a tumor , linked to a ` triggering ' arm that is specific for a molecule capable of mediating a phagocytic or lytic response by macrophages , natural killer cells , T-cells or other effector cells .
	manualset3
172785	8	413442	7	NULL	NULL	0	NULL	phagocytic response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These bispecific antibodies consist of a ` targeting ' domain , typically a fragment of a monoclonal antibody that binds to a tumor , linked to a ` triggering ' arm that is specific for a molecule capable of mediating a phagocytic or lytic response by macrophages , natural killer cells , T-cells or other effector cells .
	manualset3
172786	9	413442	7	NULL	NULL	0	NULL	 lytic response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These bispecific antibodies consist of a ` targeting ' domain , typically a fragment of a monoclonal antibody that binds to a tumor , linked to a ` triggering ' arm that is specific for a molecule capable of mediating a phagocytic or lytic response by macrophages , natural killer cells , T-cells or other effector cells .
	manualset3
172787	10	413442	7	NULL	NULL	0	NULL	macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These bispecific antibodies consist of a ` targeting ' domain , typically a fragment of a monoclonal antibody that binds to a tumor , linked to a ` triggering ' arm that is specific for a molecule capable of mediating a phagocytic or lytic response by macrophages , natural killer cells , T-cells or other effector cells .
	manualset3
172788	11	413442	7	NULL	NULL	0	NULL	natural killer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These bispecific antibodies consist of a ` targeting ' domain , typically a fragment of a monoclonal antibody that binds to a tumor , linked to a ` triggering ' arm that is specific for a molecule capable of mediating a phagocytic or lytic response by macrophages , natural killer cells , T-cells or other effector cells .
	manualset3
172789	12	413442	7	NULL	NULL	0	NULL	T-cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These bispecific antibodies consist of a ` targeting ' domain , typically a fragment of a monoclonal antibody that binds to a tumor , linked to a ` triggering ' arm that is specific for a molecule capable of mediating a phagocytic or lytic response by macrophages , natural killer cells , T-cells or other effector cells .
	manualset3
172790	13	413442	7	NULL	NULL	0	NULL	effector cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These bispecific antibodies consist of a ` targeting ' domain , typically a fragment of a monoclonal antibody that binds to a tumor , linked to a ` triggering ' arm that is specific for a molecule capable of mediating a phagocytic or lytic response by macrophages , natural killer cells , T-cells or other effector cells .
	manualset3
172791	1	413443	7	NULL	NULL	0	NULL	cDNAs 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These cDNAs encode the entire 430-amino acid sequence of pLCAD , including the 30-amino acid leader peptide and the 400-amino acid mature LCAD .
	manualset3
172792	2	413443	7	NULL	NULL	0	NULL	430-amino acid sequence	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These cDNAs encode the entire 430-amino acid sequence of pLCAD , including the 30-amino acid leader peptide and the 400-amino acid mature LCAD .
	manualset3
172793	3	413443	7	NULL	NULL	0	NULL	pLCAD	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These cDNAs encode the entire 430-amino acid sequence of pLCAD , including the 30-amino acid leader peptide and the 400-amino acid mature LCAD .
	manualset3
172794	4	413443	7	NULL	NULL	0	NULL	30-amino acid leader peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	These cDNAs encode the entire 430-amino acid sequence of pLCAD , including the 30-amino acid leader peptide and the 400-amino acid mature LCAD .
	manualset3
172795	5	413443	7	NULL	NULL	0	NULL	 400-amino acid	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These cDNAs encode the entire 430-amino acid sequence of pLCAD , including the 30-amino acid leader peptide and the 400-amino acid mature LCAD .
	manualset3
172796	6	413443	7	NULL	NULL	0	NULL	LCAD	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These cDNAs encode the entire 430-amino acid sequence of pLCAD , including the 30-amino acid leader peptide and the 400-amino acid mature LCAD .
	manualset3
172797	1	413444	7	NULL	NULL	0	NULL	 cDNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These cDNAs yielded proteins that comigrate with the native isoforms , cTnT1 through cTnT4 .
	manualset3
172798	2	413444	7	NULL	NULL	0	NULL	proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These cDNAs yielded proteins that comigrate with the native isoforms , cTnT1 through cTnT4 .
	manualset3
172799	3	413444	7	NULL	NULL	0	NULL	native isoforms	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These cDNAs yielded proteins that comigrate with the native isoforms , cTnT1 through cTnT4 .
	manualset3
172800	4	413444	7	NULL	NULL	0	NULL	cTnT1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These cDNAs yielded proteins that comigrate with the native isoforms , cTnT1 through cTnT4 .
	manualset3
172801	5	413444	7	NULL	NULL	0	NULL	cTnT4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These cDNAs yielded proteins that comigrate with the native isoforms , cTnT1 through cTnT4 .
	manualset3
172802	1	413445	7	NULL	NULL	0	NULL	calli	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These calli were co-cultured with A. tumefaciens harboring a plasmid vector containing the H. brasiliensis superoxide dismutase gene ( HbSOD ) under the control of the CaMV 35S promoter .
	manualset3
172803	2	413445	7	NULL	NULL	0	NULL	A. tumefaciens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These calli were co-cultured with A. tumefaciens harboring a plasmid vector containing the H. brasiliensis superoxide dismutase gene ( HbSOD ) under the control of the CaMV 35S promoter .
	manualset3
172804	3	413445	7	NULL	NULL	0	NULL	plasmid vector	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These calli were co-cultured with A. tumefaciens harboring a plasmid vector containing the H. brasiliensis superoxide dismutase gene ( HbSOD ) under the control of the CaMV 35S promoter .
	manualset3
172805	4	413445	7	NULL	NULL	0	NULL	H. brasiliensis superoxide dismutase gene ( HbSOD )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	These calli were co-cultured with A. tumefaciens harboring a plasmid vector containing the H. brasiliensis superoxide dismutase gene ( HbSOD ) under the control of the CaMV 35S promoter .
	manualset3
172806	5	413445	7	NULL	NULL	0	NULL	control 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These calli were co-cultured with A. tumefaciens harboring a plasmid vector containing the H. brasiliensis superoxide dismutase gene ( HbSOD ) under the control of the CaMV 35S promoter .
	manualset3
172807	6	413445	7	NULL	NULL	0	NULL	CaMV 35S promoter 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These calli were co-cultured with A. tumefaciens harboring a plasmid vector containing the H. brasiliensis superoxide dismutase gene ( HbSOD ) under the control of the CaMV 35S promoter .
	manualset3
173005	1	413446	7	NULL	NULL	0	NULL	depletion interaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These can be attributed to the depletion interaction , which results in an effective attraction between the two proteins , winning over the repulsive force .
	manualset3
173006	2	413446	7	NULL	NULL	0	NULL	effective attraction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These can be attributed to the depletion interaction , which results in an effective attraction between the two proteins , winning over the repulsive force .
	manualset3
173007	3	413446	7	NULL	NULL	0	NULL	 two proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These can be attributed to the depletion interaction , which results in an effective attraction between the two proteins , winning over the repulsive force .
	manualset3
173008	4	413446	7	NULL	NULL	0	NULL	repulsive force	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These can be attributed to the depletion interaction , which results in an effective attraction between the two proteins , winning over the repulsive force .
	manualset3
173009	1	413447	7	NULL	NULL	0	NULL	Acute intracerebroventricular administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute intracerebroventricular administration of TLQP-21 decreased food intake , and chronic treatment caused a sustained reduction in food intake and body weight and decreased abdominal fat depots .
	manualset3
173010	2	413447	7	NULL	NULL	0	NULL	TLQP-21	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute intracerebroventricular administration of TLQP-21 decreased food intake , and chronic treatment caused a sustained reduction in food intake and body weight and decreased abdominal fat depots .
	manualset3
173011	3	413447	7	NULL	NULL	0	NULL	food intake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute intracerebroventricular administration of TLQP-21 decreased food intake , and chronic treatment caused a sustained reduction in food intake and body weight and decreased abdominal fat depots .
	manualset3
173012	4	413447	7	NULL	NULL	0	NULL	chronic treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute intracerebroventricular administration of TLQP-21 decreased food intake , and chronic treatment caused a sustained reduction in food intake and body weight and decreased abdominal fat depots .
	manualset3
173013	5	413447	7	NULL	NULL	0	NULL	reduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute intracerebroventricular administration of TLQP-21 decreased food intake , and chronic treatment caused a sustained reduction in food intake and body weight and decreased abdominal fat depots .
	manualset3
173014	6	413447	7	NULL	NULL	0	NULL	food intake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute intracerebroventricular administration of TLQP-21 decreased food intake , and chronic treatment caused a sustained reduction in food intake and body weight and decreased abdominal fat depots .
	manualset3
173015	7	413447	7	NULL	NULL	0	NULL	body weight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute intracerebroventricular administration of TLQP-21 decreased food intake , and chronic treatment caused a sustained reduction in food intake and body weight and decreased abdominal fat depots .
	manualset3
173016	8	413447	7	NULL	NULL	0	NULL	abdominal fat depots	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute intracerebroventricular administration of TLQP-21 decreased food intake , and chronic treatment caused a sustained reduction in food intake and body weight and decreased abdominal fat depots .
	manualset3
173017	1	413448	7	NULL	NULL	0	NULL	 cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These cases illustrate the clinical , electrocardiographic and evolutive diversity of viral myocarditis .
	manualset3
173018	2	413448	7	NULL	NULL	0	NULL	clinical diversity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These cases illustrate the clinical , electrocardiographic and evolutive diversity of viral myocarditis .
	manualset3
173019	3	413448	7	NULL	NULL	0	NULL	 electrocardiographic diversity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These cases illustrate the clinical , electrocardiographic and evolutive diversity of viral myocarditis .
	manualset3
173020	4	413448	7	NULL	NULL	0	NULL	evolutive diversity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These cases illustrate the clinical , electrocardiographic and evolutive diversity of viral myocarditis .
	manualset3
173021	5	413448	7	NULL	NULL	0	NULL	viral myocarditis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These cases illustrate the clinical , electrocardiographic and evolutive diversity of viral myocarditis .
	manualset3
173022	1	413449	7	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These cases reinforce the importance of triple assessment in any woman presenting with a breast lump , even with a clear history of trauma .
	manualset3
173023	2	413449	7	NULL	NULL	0	NULL	triple assessment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These cases reinforce the importance of triple assessment in any woman presenting with a breast lump , even with a clear history of trauma .
	manualset3
173024	3	413449	7	NULL	NULL	0	NULL	woman	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	These cases reinforce the importance of triple assessment in any woman presenting with a breast lump , even with a clear history of trauma .
	manualset3
173025	4	413449	7	NULL	NULL	0	NULL	breast lump	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These cases reinforce the importance of triple assessment in any woman presenting with a breast lump , even with a clear history of trauma .
	manualset3
173026	5	413449	7	NULL	NULL	0	NULL	clear history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These cases reinforce the importance of triple assessment in any woman presenting with a breast lump , even with a clear history of trauma .
	manualset3
173027	6	413449	7	NULL	NULL	0	NULL	trauma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These cases reinforce the importance of triple assessment in any woman presenting with a breast lump , even with a clear history of trauma .
	manualset3
190508	7	413449	7	NULL	NULL	0	NULL	importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These cases reinforce the importance of triple assessment in any woman presenting with a breast lump , even with a clear history of trauma .
	manualset3
173028	1	413450	7	NULL	NULL	0	NULL	 cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These cases support the hypothesis that testicular descent is guided by the tail of the epididymis .
	manualset3
173029	2	413450	7	NULL	NULL	0	NULL	hypothesis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These cases support the hypothesis that testicular descent is guided by the tail of the epididymis .
	manualset3
173030	3	413450	7	NULL	NULL	0	NULL	testicular descent	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These cases support the hypothesis that testicular descent is guided by the tail of the epididymis .
	manualset3
173031	4	413450	7	NULL	NULL	0	NULL	 tail 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These cases support the hypothesis that testicular descent is guided by the tail of the epididymis .
	manualset3
173032	5	413450	7	NULL	NULL	0	NULL	epididymis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These cases support the hypothesis that testicular descent is guided by the tail of the epididymis .
	manualset3
173033	1	413451	7	NULL	NULL	0	NULL	categories	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These categories include patients with Joint National Committee Stage 2 , Stage 3 , or drug-resistant hypertension ; hypertension , and spontaneous or diuretic-induced hypokalemia ; hypertension with adrenal incidentaloma ; hypertension and a family history of early-onset hypertension or cerebrovascular accident at a young age and all hypertensive first degree relatives of patients with PA. .
	manualset3
173034	2	413451	7	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These categories include patients with Joint National Committee Stage 2 , Stage 3 , or drug-resistant hypertension ; hypertension , and spontaneous or diuretic-induced hypokalemia ; hypertension with adrenal incidentaloma ; hypertension and a family history of early-onset hypertension or cerebrovascular accident at a young age and all hypertensive first degree relatives of patients with PA. .
	manualset3
173035	3	413451	7	NULL	NULL	0	NULL	Joint National Committee Stage 2 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	These categories include patients with Joint National Committee Stage 2 , Stage 3 , or drug-resistant hypertension ; hypertension , and spontaneous or diuretic-induced hypokalemia ; hypertension with adrenal incidentaloma ; hypertension and a family history of early-onset hypertension or cerebrovascular accident at a young age and all hypertensive first degree relatives of patients with PA. .
	manualset3
173036	4	413451	7	NULL	NULL	0	NULL	 Stage 3	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	These categories include patients with Joint National Committee Stage 2 , Stage 3 , or drug-resistant hypertension ; hypertension , and spontaneous or diuretic-induced hypokalemia ; hypertension with adrenal incidentaloma ; hypertension and a family history of early-onset hypertension or cerebrovascular accident at a young age and all hypertensive first degree relatives of patients with PA. .
	manualset3
173037	5	413451	7	NULL	NULL	0	NULL	drug-resistant hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These categories include patients with Joint National Committee Stage 2 , Stage 3 , or drug-resistant hypertension ; hypertension , and spontaneous or diuretic-induced hypokalemia ; hypertension with adrenal incidentaloma ; hypertension and a family history of early-onset hypertension or cerebrovascular accident at a young age and all hypertensive first degree relatives of patients with PA. .
	manualset3
173038	6	413451	7	NULL	NULL	0	NULL	hypertension	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These categories include patients with Joint National Committee Stage 2 , Stage 3 , or drug-resistant hypertension ; hypertension , and spontaneous or diuretic-induced hypokalemia ; hypertension with adrenal incidentaloma ; hypertension and a family history of early-onset hypertension or cerebrovascular accident at a young age and all hypertensive first degree relatives of patients with PA. .
	manualset3
173039	7	413451	7	NULL	NULL	0	NULL	spontaneous or diuretic-induced hypokalemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These categories include patients with Joint National Committee Stage 2 , Stage 3 , or drug-resistant hypertension ; hypertension , and spontaneous or diuretic-induced hypokalemia ; hypertension with adrenal incidentaloma ; hypertension and a family history of early-onset hypertension or cerebrovascular accident at a young age and all hypertensive first degree relatives of patients with PA. .
	manualset3
173040	8	413451	7	NULL	NULL	0	NULL	hypertension with adrenal incidentaloma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These categories include patients with Joint National Committee Stage 2 , Stage 3 , or drug-resistant hypertension ; hypertension , and spontaneous or diuretic-induced hypokalemia ; hypertension with adrenal incidentaloma ; hypertension and a family history of early-onset hypertension or cerebrovascular accident at a young age and all hypertensive first degree relatives of patients with PA. .
	manualset3
173041	9	413451	7	NULL	NULL	0	NULL	 hypertension	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These categories include patients with Joint National Committee Stage 2 , Stage 3 , or drug-resistant hypertension ; hypertension , and spontaneous or diuretic-induced hypokalemia ; hypertension with adrenal incidentaloma ; hypertension and a family history of early-onset hypertension or cerebrovascular accident at a young age and all hypertensive first degree relatives of patients with PA. .
	manualset3
173042	10	413451	7	NULL	NULL	0	NULL	 family history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These categories include patients with Joint National Committee Stage 2 , Stage 3 , or drug-resistant hypertension ; hypertension , and spontaneous or diuretic-induced hypokalemia ; hypertension with adrenal incidentaloma ; hypertension and a family history of early-onset hypertension or cerebrovascular accident at a young age and all hypertensive first degree relatives of patients with PA. .
	manualset3
173043	11	413451	7	NULL	NULL	0	NULL	 early-onset hypertension	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These categories include patients with Joint National Committee Stage 2 , Stage 3 , or drug-resistant hypertension ; hypertension , and spontaneous or diuretic-induced hypokalemia ; hypertension with adrenal incidentaloma ; hypertension and a family history of early-onset hypertension or cerebrovascular accident at a young age and all hypertensive first degree relatives of patients with PA. .
	manualset3
173044	12	413451	7	NULL	NULL	0	NULL	cerebrovascular accident 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These categories include patients with Joint National Committee Stage 2 , Stage 3 , or drug-resistant hypertension ; hypertension , and spontaneous or diuretic-induced hypokalemia ; hypertension with adrenal incidentaloma ; hypertension and a family history of early-onset hypertension or cerebrovascular accident at a young age and all hypertensive first degree relatives of patients with PA. .
	manualset3
173045	13	413451	7	NULL	NULL	NULL	NULL	young age	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These categories include patients with Joint National Committee Stage 2 , Stage 3 , or drug-resistant hypertension ; hypertension , and spontaneous or diuretic-induced hypokalemia ; hypertension with adrenal incidentaloma ; hypertension and a family history of early-onset hypertension or cerebrovascular accident at a young age and all hypertensive first degree relatives of patients with PA. .
	manualset3
173046	14	413451	7	NULL	NULL	0	NULL	hypertensive first degree relatives	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These categories include patients with Joint National Committee Stage 2 , Stage 3 , or drug-resistant hypertension ; hypertension , and spontaneous or diuretic-induced hypokalemia ; hypertension with adrenal incidentaloma ; hypertension and a family history of early-onset hypertension or cerebrovascular accident at a young age and all hypertensive first degree relatives of patients with PA. .
	manualset3
173047	15	413451	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These categories include patients with Joint National Committee Stage 2 , Stage 3 , or drug-resistant hypertension ; hypertension , and spontaneous or diuretic-induced hypokalemia ; hypertension with adrenal incidentaloma ; hypertension and a family history of early-onset hypertension or cerebrovascular accident at a young age and all hypertensive first degree relatives of patients with PA. .
	manualset3
173048	16	413451	7	NULL	NULL	0	NULL	PA	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These categories include patients with Joint National Committee Stage 2 , Stage 3 , or drug-resistant hypertension ; hypertension , and spontaneous or diuretic-induced hypokalemia ; hypertension with adrenal incidentaloma ; hypertension and a family history of early-onset hypertension or cerebrovascular accident at a young age and all hypertensive first degree relatives of patients with PA. .
	manualset3
173049	1	413452	7	NULL	NULL	0	NULL	cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These cell lines were treated with TS leaf extract and screened for viability , apoptosis , necrosis , and apoptotic gene expression .
	manualset3
173050	2	413452	7	NULL	NULL	0	NULL	TS leaf extract 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These cell lines were treated with TS leaf extract and screened for viability , apoptosis , necrosis , and apoptotic gene expression .
	manualset3
173051	3	413452	7	NULL	NULL	NULL	NULL	viability	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These cell lines were treated with TS leaf extract and screened for viability , apoptosis , necrosis , and apoptotic gene expression .
	manualset3
173052	4	413452	7	NULL	NULL	NULL	NULL	apoptosis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These cell lines were treated with TS leaf extract and screened for viability , apoptosis , necrosis , and apoptotic gene expression .
	manualset3
173053	5	413452	7	NULL	NULL	NULL	NULL	necrosis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These cell lines were treated with TS leaf extract and screened for viability , apoptosis , necrosis , and apoptotic gene expression .
	manualset3
173054	6	413452	7	NULL	NULL	0	NULL	apoptotic gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These cell lines were treated with TS leaf extract and screened for viability , apoptosis , necrosis , and apoptotic gene expression .
	manualset3
173055	1	413453	7	NULL	NULL	0	NULL	cell types	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These cell types release proinflammatory cytokines and cytotoxic mediators to destroy invading pathogens and initiate wound repair .
	manualset3
173056	2	413453	7	NULL	NULL	0	NULL	proinflammatory cytokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These cell types release proinflammatory cytokines and cytotoxic mediators to destroy invading pathogens and initiate wound repair .
	manualset3
173057	3	413453	7	NULL	NULL	0	NULL	cytotoxic mediators	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These cell types release proinflammatory cytokines and cytotoxic mediators to destroy invading pathogens and initiate wound repair .
	manualset3
173058	4	413453	7	NULL	NULL	0	NULL	pathogens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These cell types release proinflammatory cytokines and cytotoxic mediators to destroy invading pathogens and initiate wound repair .
	manualset3
173059	5	413453	7	NULL	NULL	0	NULL	wound repair 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These cell types release proinflammatory cytokines and cytotoxic mediators to destroy invading pathogens and initiate wound repair .
	manualset3
173060	1	413454	7	NULL	NULL	0	NULL	 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These cells do not emit projection axons , a characteristic that bespeaks against these cells being considered as pioneer neurons .
	manualset3
173061	2	413454	7	NULL	NULL	0	NULL	projection axons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These cells do not emit projection axons , a characteristic that bespeaks against these cells being considered as pioneer neurons .
	manualset3
173062	3	413454	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These cells do not emit projection axons , a characteristic that bespeaks against these cells being considered as pioneer neurons .
	manualset3
173063	4	413454	7	NULL	NULL	0	NULL	neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These cells do not emit projection axons , a characteristic that bespeaks against these cells being considered as pioneer neurons .
	manualset3
173064	1	413455	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These cells express CTLA-4 and glucocorticoid-induced TNR receptor and inhibit T cell proliferation in a contact-dependent manner .
	manualset3
173065	2	413455	7	NULL	NULL	0	NULL	CTLA-4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These cells express CTLA-4 and glucocorticoid-induced TNR receptor and inhibit T cell proliferation in a contact-dependent manner .
	manualset3
173066	3	413455	7	NULL	NULL	0	NULL	 glucocorticoid-induced TNR receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These cells express CTLA-4 and glucocorticoid-induced TNR receptor and inhibit T cell proliferation in a contact-dependent manner .
	manualset3
173067	4	413455	7	NULL	NULL	0	NULL	T cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These cells express CTLA-4 and glucocorticoid-induced TNR receptor and inhibit T cell proliferation in a contact-dependent manner .
	manualset3
173068	5	413455	7	NULL	NULL	0	NULL	contact-dependent manner	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These cells express CTLA-4 and glucocorticoid-induced TNR receptor and inhibit T cell proliferation in a contact-dependent manner .
	manualset3
173069	1	413456	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These cells have been shown to contain ryanodine receptor ( Zupanc et al. , 1992 ) .
	manualset3
173070	2	413456	7	NULL	NULL	0	NULL	 ryanodine receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These cells have been shown to contain ryanodine receptor ( Zupanc et al. , 1992 ) .
	manualset3
173071	3	413456	7	NULL	NULL	0	NULL	Zupanc et al. , 1992	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	These cells have been shown to contain ryanodine receptor ( Zupanc et al. , 1992 ) .
	manualset3
173072	1	413457	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These cells were used as a model to assess the regulation of flotillin-1 mRNA and protein expression by cell-cell interactions .
	manualset3
173073	2	413457	7	NULL	NULL	0	NULL	 model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These cells were used as a model to assess the regulation of flotillin-1 mRNA and protein expression by cell-cell interactions .
	manualset3
173074	3	413457	7	NULL	NULL	0	NULL	regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These cells were used as a model to assess the regulation of flotillin-1 mRNA and protein expression by cell-cell interactions .
	manualset3
173075	4	413457	7	NULL	NULL	0	NULL	flotillin-1 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These cells were used as a model to assess the regulation of flotillin-1 mRNA and protein expression by cell-cell interactions .
	manualset3
173076	5	413457	7	NULL	NULL	0	NULL	protein expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These cells were used as a model to assess the regulation of flotillin-1 mRNA and protein expression by cell-cell interactions .
	manualset3
173077	6	413457	7	NULL	NULL	0	NULL	cell-cell interactions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These cells were used as a model to assess the regulation of flotillin-1 mRNA and protein expression by cell-cell interactions .
	manualset3
173078	1	413458	7	NULL	NULL	0	NULL	 changes 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These changes in distance are consistent with a flattening of propellor twist of the AT base-pairs .
	manualset3
173079	2	413458	7	NULL	NULL	0	NULL	distance 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These changes in distance are consistent with a flattening of propellor twist of the AT base-pairs .
	manualset3
173080	3	413458	7	NULL	NULL	0	NULL	flattening 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These changes in distance are consistent with a flattening of propellor twist of the AT base-pairs .
	manualset3
173081	4	413458	7	NULL	NULL	0	NULL	propellor twist 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These changes in distance are consistent with a flattening of propellor twist of the AT base-pairs .
	manualset3
173082	5	413458	7	NULL	NULL	0	NULL	AT base-pairs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These changes in distance are consistent with a flattening of propellor twist of the AT base-pairs .
	manualset3
173083	1	413459	7	NULL	NULL	0	NULL	changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These changes were inhibited by phenylarsine oxide and are likely to involve the same channel that is involved in the response to ABA .
	manualset3
173084	2	413459	7	NULL	NULL	0	NULL	phenylarsine oxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These changes were inhibited by phenylarsine oxide and are likely to involve the same channel that is involved in the response to ABA .
	manualset3
173085	3	413459	7	NULL	NULL	0	NULL	channel	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These changes were inhibited by phenylarsine oxide and are likely to involve the same channel that is involved in the response to ABA .
	manualset3
173086	4	413459	7	NULL	NULL	0	NULL	response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These changes were inhibited by phenylarsine oxide and are likely to involve the same channel that is involved in the response to ABA .
	manualset3
173087	5	413459	7	NULL	NULL	0	NULL	ABA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These changes were inhibited by phenylarsine oxide and are likely to involve the same channel that is involved in the response to ABA .
	manualset3
173088	1	413460	7	NULL	NULL	0	NULL	Acute myocardial infarction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute myocardial infarction due to aortic dissection .
	manualset3
173089	2	413460	7	NULL	NULL	0	NULL	aortic dissection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute myocardial infarction due to aortic dissection .
	manualset3
173090	1	413461	7	NULL	NULL	0	NULL	characteristics	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These characteristics are also observed in the cells of the `` dermatome '' layer of the dermo-myotome ; and so , it appears probable that the cells of the `` dermatome '' .
	manualset3
173091	2	413461	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These characteristics are also observed in the cells of the `` dermatome '' layer of the dermo-myotome ; and so , it appears probable that the cells of the `` dermatome '' .
	manualset3
173092	3	413461	7	NULL	NULL	NULL	NULL	 `` dermatome '' layer 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These characteristics are also observed in the cells of the `` dermatome '' layer of the dermo-myotome ; and so , it appears probable that the cells of the `` dermatome '' .
	manualset3
173093	4	413461	7	NULL	NULL	NULL	NULL	dermo-myotome	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These characteristics are also observed in the cells of the `` dermatome '' layer of the dermo-myotome ; and so , it appears probable that the cells of the `` dermatome '' .
	manualset3
173094	5	413461	7	NULL	NULL	0	NULL	 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These characteristics are also observed in the cells of the `` dermatome '' layer of the dermo-myotome ; and so , it appears probable that the cells of the `` dermatome '' .
	manualset3
173095	6	413461	7	NULL	NULL	0	NULL	dermatome	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These characteristics are also observed in the cells of the `` dermatome '' layer of the dermo-myotome ; and so , it appears probable that the cells of the `` dermatome '' .
	manualset3
173096	1	413462	7	NULL	NULL	0	NULL	characteristics	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These characteristics may induce to an inapropiated diagnosis of malignant neoplasia .
	manualset3
173097	2	413462	7	NULL	NULL	NULL	NULL	 diagnosis	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These characteristics may induce to an inapropiated diagnosis of malignant neoplasia .
	manualset3
173098	3	413462	7	NULL	NULL	NULL	NULL	malignant neoplasia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These characteristics may induce to an inapropiated diagnosis of malignant neoplasia .
	manualset3
173099	1	413463	7	NULL	NULL	0	NULL	characteristics 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These characteristics of the transduction mechanisms may be related to the immature state of the eel gonadotrophs at the silver stage .
	manualset3
173100	2	413463	7	NULL	NULL	0	NULL	 transduction mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These characteristics of the transduction mechanisms may be related to the immature state of the eel gonadotrophs at the silver stage .
	manualset3
173101	3	413463	7	NULL	NULL	NULL	NULL	 immature state 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These characteristics of the transduction mechanisms may be related to the immature state of the eel gonadotrophs at the silver stage .
	manualset3
173102	4	413463	7	NULL	NULL	0	NULL	eel gonadotrophs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These characteristics of the transduction mechanisms may be related to the immature state of the eel gonadotrophs at the silver stage .
	manualset3
173103	5	413463	7	NULL	NULL	0	NULL	silver stage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These characteristics of the transduction mechanisms may be related to the immature state of the eel gonadotrophs at the silver stage .
	manualset3
173104	1	413464	7	NULL	NULL	0	NULL	chlorellae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These chlorellae tolerate wide ranges of acidity and temperature ; they both grow and form cysts in media in which sodium ions are replaced with potassium .
	manualset3
173105	2	413464	7	NULL	NULL	0	NULL	ranges 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These chlorellae tolerate wide ranges of acidity and temperature ; they both grow and form cysts in media in which sodium ions are replaced with potassium .
	manualset3
173106	3	413464	7	NULL	NULL	0	NULL	acidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These chlorellae tolerate wide ranges of acidity and temperature ; they both grow and form cysts in media in which sodium ions are replaced with potassium .
	manualset3
173107	4	413464	7	NULL	NULL	0	NULL	temperature	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These chlorellae tolerate wide ranges of acidity and temperature ; they both grow and form cysts in media in which sodium ions are replaced with potassium .
	manualset3
173108	5	413464	7	NULL	NULL	0	NULL	grow 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These chlorellae tolerate wide ranges of acidity and temperature ; they both grow and form cysts in media in which sodium ions are replaced with potassium .
	manualset3
173109	6	413464	7	NULL	NULL	0	NULL	cysts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These chlorellae tolerate wide ranges of acidity and temperature ; they both grow and form cysts in media in which sodium ions are replaced with potassium .
	manualset3
173110	7	413464	7	NULL	NULL	0	NULL	media	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These chlorellae tolerate wide ranges of acidity and temperature ; they both grow and form cysts in media in which sodium ions are replaced with potassium .
	manualset3
173111	8	413464	7	NULL	NULL	0	NULL	sodium ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	These chlorellae tolerate wide ranges of acidity and temperature ; they both grow and form cysts in media in which sodium ions are replaced with potassium .
	manualset3
173112	9	413464	7	NULL	NULL	0	NULL	potassium	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	These chlorellae tolerate wide ranges of acidity and temperature ; they both grow and form cysts in media in which sodium ions are replaced with potassium .
	manualset3
173113	1	413465	7	NULL	NULL	0	NULL	clinical parameters 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These clinical parameters showed a significant improvement after thermal mud and DAR ; tolerance of both treatments was excellent in all patients .
	manualset3
173114	2	413465	7	NULL	NULL	0	NULL	improvement	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These clinical parameters showed a significant improvement after thermal mud and DAR ; tolerance of both treatments was excellent in all patients .
	manualset3
173115	3	413465	7	NULL	NULL	0	NULL	 thermal mud	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These clinical parameters showed a significant improvement after thermal mud and DAR ; tolerance of both treatments was excellent in all patients .
	manualset3
173116	4	413465	7	NULL	NULL	0	NULL	DAR	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These clinical parameters showed a significant improvement after thermal mud and DAR ; tolerance of both treatments was excellent in all patients .
	manualset3
173117	5	413465	7	NULL	NULL	0	NULL	tolerance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These clinical parameters showed a significant improvement after thermal mud and DAR ; tolerance of both treatments was excellent in all patients .
	manualset3
173118	6	413465	7	NULL	NULL	0	NULL	treatments	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These clinical parameters showed a significant improvement after thermal mud and DAR ; tolerance of both treatments was excellent in all patients .
	manualset3
173119	7	413465	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These clinical parameters showed a significant improvement after thermal mud and DAR ; tolerance of both treatments was excellent in all patients .
	manualset3
173120	1	413466	7	NULL	NULL	0	NULL	combined results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These combined results indicate that soy isoflavones can alter early-event signaling networks that result in less activated platelets and may partially explain the beneficial effects of dietary soy against human heart disease .
	manualset3
173121	2	413466	7	NULL	NULL	0	NULL	soy isoflavones	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These combined results indicate that soy isoflavones can alter early-event signaling networks that result in less activated platelets and may partially explain the beneficial effects of dietary soy against human heart disease .
	manualset3
173122	3	413466	7	NULL	NULL	0	NULL	 early-event signaling networks	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These combined results indicate that soy isoflavones can alter early-event signaling networks that result in less activated platelets and may partially explain the beneficial effects of dietary soy against human heart disease .
	manualset3
173123	4	413466	7	NULL	NULL	0	NULL	less activated platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These combined results indicate that soy isoflavones can alter early-event signaling networks that result in less activated platelets and may partially explain the beneficial effects of dietary soy against human heart disease .
	manualset3
173124	5	413466	7	NULL	NULL	0	NULL	beneficial effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These combined results indicate that soy isoflavones can alter early-event signaling networks that result in less activated platelets and may partially explain the beneficial effects of dietary soy against human heart disease .
	manualset3
173125	6	413466	7	NULL	NULL	NULL	NULL	dietary soy 	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These combined results indicate that soy isoflavones can alter early-event signaling networks that result in less activated platelets and may partially explain the beneficial effects of dietary soy against human heart disease .
	manualset3
173126	7	413466	7	NULL	NULL	0	NULL	human heart disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These combined results indicate that soy isoflavones can alter early-event signaling networks that result in less activated platelets and may partially explain the beneficial effects of dietary soy against human heart disease .
	manualset3
173127	1	413467	7	NULL	NULL	NULL	NULL	complexes	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These complexes are formed by direct eps15-homology ( EH ) domain/asparagine proline phenylalanine ( NPF ) motif interactions .
	manualset3
173128	2	413467	7	NULL	NULL	0	NULL	direct eps15-homology ( EH ) domain/asparagine proline phenylalanine ( NPF ) motif interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These complexes are formed by direct eps15-homology ( EH ) domain/asparagine proline phenylalanine ( NPF ) motif interactions .
	manualset3
173129	1	413468	7	NULL	NULL	0	NULL	Acute onset	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute onset of dyspnea associated with colonoscopy .
	manualset3
173130	2	413468	7	NULL	NULL	0	NULL	dyspnea	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute onset of dyspnea associated with colonoscopy .
	manualset3
173131	3	413468	7	NULL	NULL	0	NULL	colonoscopy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute onset of dyspnea associated with colonoscopy .
	manualset3
173132	1	413469	7	NULL	NULL	0	NULL	complexes	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These complexes were inert to photoisomerization though the ligand itself was isomerized upon photoirradiation .
	manualset3
173133	2	413469	7	NULL	NULL	0	NULL	photoisomerization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These complexes were inert to photoisomerization though the ligand itself was isomerized upon photoirradiation .
	manualset3
173134	3	413469	7	NULL	NULL	NULL	NULL	 ligand	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These complexes were inert to photoisomerization though the ligand itself was isomerized upon photoirradiation .
	manualset3
173135	4	413469	7	NULL	NULL	0	NULL	photoirradiation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These complexes were inert to photoisomerization though the ligand itself was isomerized upon photoirradiation .
	manualset3
173136	1	413470	7	NULL	NULL	0	NULL	complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These complications from advanced-stage lung cancer can be a serious threat to life and require appropriate intervention .
	manualset3
173137	2	413470	7	NULL	NULL	0	NULL	advanced-stage lung cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These complications from advanced-stage lung cancer can be a serious threat to life and require appropriate intervention .
	manualset3
173138	3	413470	7	NULL	NULL	0	NULL	serious threat 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These complications from advanced-stage lung cancer can be a serious threat to life and require appropriate intervention .
	manualset3
173139	4	413470	7	NULL	NULL	0	NULL	 life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These complications from advanced-stage lung cancer can be a serious threat to life and require appropriate intervention .
	manualset3
173140	5	413470	7	NULL	NULL	0	NULL	 intervention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These complications from advanced-stage lung cancer can be a serious threat to life and require appropriate intervention .
	manualset3
173141	1	413471	7	NULL	NULL	0	NULL	 complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These complications may arise at any time after the institution of heparin therapy .
	manualset3
173142	2	413471	7	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	These complications may arise at any time after the institution of heparin therapy .
	manualset3
173143	3	413471	7	NULL	NULL	0	NULL	 institution	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These complications may arise at any time after the institution of heparin therapy .
	manualset3
173144	4	413471	7	NULL	NULL	0	NULL	heparin therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These complications may arise at any time after the institution of heparin therapy .
	manualset3
173145	1	413472	7	NULL	NULL	0	NULL	 compounds	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These compounds , together with their related enzymes , that include key proteins for the synthesis and degradation of endocannabinoids , cannabinoid and non-cannabinoid receptors , and purported membrane transporter ( s ) , form the `` endocannabinoid system ( ECS ) '' .
	manualset3
173146	2	413472	7	NULL	NULL	0	NULL	enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These compounds , together with their related enzymes , that include key proteins for the synthesis and degradation of endocannabinoids , cannabinoid and non-cannabinoid receptors , and purported membrane transporter ( s ) , form the `` endocannabinoid system ( ECS ) '' .
	manualset3
173147	3	413472	7	NULL	NULL	0	NULL	proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These compounds , together with their related enzymes , that include key proteins for the synthesis and degradation of endocannabinoids , cannabinoid and non-cannabinoid receptors , and purported membrane transporter ( s ) , form the `` endocannabinoid system ( ECS ) '' .
	manualset3
173148	4	413472	7	NULL	NULL	0	NULL	synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These compounds , together with their related enzymes , that include key proteins for the synthesis and degradation of endocannabinoids , cannabinoid and non-cannabinoid receptors , and purported membrane transporter ( s ) , form the `` endocannabinoid system ( ECS ) '' .
	manualset3
173149	5	413472	7	NULL	NULL	0	NULL	degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These compounds , together with their related enzymes , that include key proteins for the synthesis and degradation of endocannabinoids , cannabinoid and non-cannabinoid receptors , and purported membrane transporter ( s ) , form the `` endocannabinoid system ( ECS ) '' .
	manualset3
173150	6	413472	7	NULL	NULL	0	NULL	endocannabinoids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These compounds , together with their related enzymes , that include key proteins for the synthesis and degradation of endocannabinoids , cannabinoid and non-cannabinoid receptors , and purported membrane transporter ( s ) , form the `` endocannabinoid system ( ECS ) '' .
	manualset3
173151	7	413472	7	NULL	NULL	NULL	NULL	 cannabinoid and non-cannabinoid receptors	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These compounds , together with their related enzymes , that include key proteins for the synthesis and degradation of endocannabinoids , cannabinoid and non-cannabinoid receptors , and purported membrane transporter ( s ) , form the `` endocannabinoid system ( ECS ) '' .
	manualset3
173152	8	413472	7	NULL	NULL	NULL	NULL	membrane transporter ( s )	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These compounds , together with their related enzymes , that include key proteins for the synthesis and degradation of endocannabinoids , cannabinoid and non-cannabinoid receptors , and purported membrane transporter ( s ) , form the `` endocannabinoid system ( ECS ) '' .
	manualset3
173153	9	413472	7	NULL	NULL	0	NULL	`` endocannabinoid system ( ECS ) ''	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These compounds , together with their related enzymes , that include key proteins for the synthesis and degradation of endocannabinoids , cannabinoid and non-cannabinoid receptors , and purported membrane transporter ( s ) , form the `` endocannabinoid system ( ECS ) '' .
	manualset3
173154	1	413473	7	NULL	NULL	0	NULL	compounds 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These compounds differ from the said drugs in having a 3 , 8-diazabicyclo ( 3 , 2 , 1 ) octane as a basic moiety .
	manualset3
173155	2	413473	7	NULL	NULL	0	NULL	 drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These compounds differ from the said drugs in having a 3 , 8-diazabicyclo ( 3 , 2 , 1 ) octane as a basic moiety .
	manualset3
173156	3	413473	7	NULL	NULL	0	NULL	3 , 8-diazabicyclo ( 3 , 2 , 1 ) octane	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These compounds differ from the said drugs in having a 3 , 8-diazabicyclo ( 3 , 2 , 1 ) octane as a basic moiety .
	manualset3
173157	4	413473	7	NULL	NULL	0	NULL	basic moiety	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These compounds differ from the said drugs in having a 3 , 8-diazabicyclo ( 3 , 2 , 1 ) octane as a basic moiety .
	manualset3
173158	1	413474	7	NULL	NULL	NULL	NULL	compounds	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These compounds induced pH equilibration in liposomes loaded with the pH probe pyranine .
	manualset3
173159	2	413474	7	NULL	NULL	0	NULL	pH equilibration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These compounds induced pH equilibration in liposomes loaded with the pH probe pyranine .
	manualset3
173160	3	413474	7	NULL	NULL	0	NULL	liposomes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These compounds induced pH equilibration in liposomes loaded with the pH probe pyranine .
	manualset3
173161	4	413474	7	NULL	NULL	0	NULL	pH probe pyranine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These compounds induced pH equilibration in liposomes loaded with the pH probe pyranine .
	manualset3
173162	1	413475	7	NULL	NULL	NULL	NULL	 compounds	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These compounds showed lethal activity against the mpk1Delta strain , specifically , compared to the cnb1Delta strain , and ion-sensitive activity against the wild-type strain in the presence of LiCl , indicating that their molecular target might be the calcineurin pathway .
	manualset3
173163	2	413475	7	NULL	NULL	0	NULL	lethal activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These compounds showed lethal activity against the mpk1Delta strain , specifically , compared to the cnb1Delta strain , and ion-sensitive activity against the wild-type strain in the presence of LiCl , indicating that their molecular target might be the calcineurin pathway .
	manualset3
173164	3	413475	7	NULL	NULL	0	NULL	mpk1Delta strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These compounds showed lethal activity against the mpk1Delta strain , specifically , compared to the cnb1Delta strain , and ion-sensitive activity against the wild-type strain in the presence of LiCl , indicating that their molecular target might be the calcineurin pathway .
	manualset3
173165	4	413475	7	NULL	NULL	0	NULL	cnb1Delta strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These compounds showed lethal activity against the mpk1Delta strain , specifically , compared to the cnb1Delta strain , and ion-sensitive activity against the wild-type strain in the presence of LiCl , indicating that their molecular target might be the calcineurin pathway .
	manualset3
173166	5	413475	7	NULL	NULL	0	NULL	ion-sensitive activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These compounds showed lethal activity against the mpk1Delta strain , specifically , compared to the cnb1Delta strain , and ion-sensitive activity against the wild-type strain in the presence of LiCl , indicating that their molecular target might be the calcineurin pathway .
	manualset3
173167	6	413475	7	NULL	NULL	0	NULL	wild-type strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These compounds showed lethal activity against the mpk1Delta strain , specifically , compared to the cnb1Delta strain , and ion-sensitive activity against the wild-type strain in the presence of LiCl , indicating that their molecular target might be the calcineurin pathway .
	manualset3
173168	7	413475	7	NULL	NULL	0	NULL	 presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These compounds showed lethal activity against the mpk1Delta strain , specifically , compared to the cnb1Delta strain , and ion-sensitive activity against the wild-type strain in the presence of LiCl , indicating that their molecular target might be the calcineurin pathway .
	manualset3
173169	8	413475	7	NULL	NULL	0	NULL	LiCl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These compounds showed lethal activity against the mpk1Delta strain , specifically , compared to the cnb1Delta strain , and ion-sensitive activity against the wild-type strain in the presence of LiCl , indicating that their molecular target might be the calcineurin pathway .
	manualset3
173170	9	413475	7	NULL	NULL	0	NULL	molecular target	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These compounds showed lethal activity against the mpk1Delta strain , specifically , compared to the cnb1Delta strain , and ion-sensitive activity against the wild-type strain in the presence of LiCl , indicating that their molecular target might be the calcineurin pathway .
	manualset3
173171	10	413475	7	NULL	NULL	0	NULL	calcineurin pathway 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These compounds showed lethal activity against the mpk1Delta strain , specifically , compared to the cnb1Delta strain , and ion-sensitive activity against the wild-type strain in the presence of LiCl , indicating that their molecular target might be the calcineurin pathway .
	manualset3
173172	1	413476	7	NULL	NULL	0	NULL	conclusions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These conclusions are illustrated here by using a series of alkyl - and halophenols .
	manualset3
173173	2	413476	7	NULL	NULL	0	NULL	series	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These conclusions are illustrated here by using a series of alkyl - and halophenols .
	manualset3
173174	3	413476	7	NULL	NULL	0	NULL	alkyl - phenols	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These conclusions are illustrated here by using a series of alkyl - and halophenols .
	manualset3
173175	4	413476	7	NULL	NULL	0	NULL	halophenols	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These conclusions are illustrated here by using a series of alkyl - and halophenols .
	manualset3
173176	1	413477	7	NULL	NULL	0	NULL	 conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These conditions should be taken into consideration during drug therapy in patients with malnutrition .
	manualset3
173177	2	413477	7	NULL	NULL	0	NULL	consideration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These conditions should be taken into consideration during drug therapy in patients with malnutrition .
	manualset3
173178	3	413477	7	NULL	NULL	0	NULL	drug therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These conditions should be taken into consideration during drug therapy in patients with malnutrition .
	manualset3
173179	4	413477	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These conditions should be taken into consideration during drug therapy in patients with malnutrition .
	manualset3
173180	5	413477	7	NULL	NULL	0	NULL	malnutrition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These conditions should be taken into consideration during drug therapy in patients with malnutrition .
	manualset3
173181	1	413478	7	NULL	NULL	0	NULL	 changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These considerable changes of the phase diagram have to be taken into account in upcoming experiments with dipolar molecules .
	manualset3
173182	2	413478	7	NULL	NULL	0	NULL	phase diagram	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These considerable changes of the phase diagram have to be taken into account in upcoming experiments with dipolar molecules .
	manualset3
173183	3	413478	7	NULL	NULL	NULL	NULL	account	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These considerable changes of the phase diagram have to be taken into account in upcoming experiments with dipolar molecules .
	manualset3
173184	4	413478	7	NULL	NULL	0	NULL	upcoming experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These considerable changes of the phase diagram have to be taken into account in upcoming experiments with dipolar molecules .
	manualset3
173185	5	413478	7	NULL	NULL	0	NULL	dipolar molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	These considerable changes of the phase diagram have to be taken into account in upcoming experiments with dipolar molecules .
	manualset3
173186	1	413479	7	NULL	NULL	0	NULL	Acute organ transplant rejection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute organ transplant rejection is characterized by a heavy lymphocyte infiltration .
	manualset3
173187	2	413479	7	NULL	NULL	0	NULL	heavy lymphocyte infiltration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute organ transplant rejection is characterized by a heavy lymphocyte infiltration .
	manualset3
173188	1	413480	7	NULL	NULL	0	NULL	constructs	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	These constructs were tested in mammalian cells to evaluate their ability to transactivate luciferase gene placed under the control of GAL4 response elements and synthetic TATAA promoter .
	manualset3
173189	2	413480	7	NULL	NULL	0	NULL	mammalian cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These constructs were tested in mammalian cells to evaluate their ability to transactivate luciferase gene placed under the control of GAL4 response elements and synthetic TATAA promoter .
	manualset3
173190	3	413480	7	NULL	NULL	NULL	NULL	ability	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These constructs were tested in mammalian cells to evaluate their ability to transactivate luciferase gene placed under the control of GAL4 response elements and synthetic TATAA promoter .
	manualset3
173191	4	413480	7	NULL	NULL	0	NULL	luciferase gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	These constructs were tested in mammalian cells to evaluate their ability to transactivate luciferase gene placed under the control of GAL4 response elements and synthetic TATAA promoter .
	manualset3
173192	5	413480	7	NULL	NULL	0	NULL	 control 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These constructs were tested in mammalian cells to evaluate their ability to transactivate luciferase gene placed under the control of GAL4 response elements and synthetic TATAA promoter .
	manualset3
173193	6	413480	7	NULL	NULL	NULL	NULL	GAL4 response elements	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These constructs were tested in mammalian cells to evaluate their ability to transactivate luciferase gene placed under the control of GAL4 response elements and synthetic TATAA promoter .
	manualset3
173194	7	413480	7	NULL	NULL	0	NULL	synthetic TATAA promoter 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These constructs were tested in mammalian cells to evaluate their ability to transactivate luciferase gene placed under the control of GAL4 response elements and synthetic TATAA promoter .
	manualset3
173195	1	413481	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data allowed us to compute an atomic model for the CP-AAA-ATPase subcomplex .
	manualset3
173196	2	413481	7	NULL	NULL	0	NULL	atomic model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These data allowed us to compute an atomic model for the CP-AAA-ATPase subcomplex .
	manualset3
173197	3	413481	7	NULL	NULL	NULL	NULL	CP-AAA-ATPase subcomplex	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data allowed us to compute an atomic model for the CP-AAA-ATPase subcomplex .
	manualset3
173198	1	413482	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data also indicate that a coordinated program of lymphoid gene expression involving TdT-CD7-expression and Ig/T beta rearrangements can be activated before myeloid commitment .
	manualset3
173199	2	413482	7	NULL	NULL	0	NULL	coordinated program 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data also indicate that a coordinated program of lymphoid gene expression involving TdT-CD7-expression and Ig/T beta rearrangements can be activated before myeloid commitment .
	manualset3
173200	3	413482	7	NULL	NULL	0	NULL	 lymphoid gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data also indicate that a coordinated program of lymphoid gene expression involving TdT-CD7-expression and Ig/T beta rearrangements can be activated before myeloid commitment .
	manualset3
173201	4	413482	7	NULL	NULL	0	NULL	TdT-CD7-expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data also indicate that a coordinated program of lymphoid gene expression involving TdT-CD7-expression and Ig/T beta rearrangements can be activated before myeloid commitment .
	manualset3
173202	5	413482	7	NULL	NULL	0	NULL	Ig/T beta rearrangements 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data also indicate that a coordinated program of lymphoid gene expression involving TdT-CD7-expression and Ig/T beta rearrangements can be activated before myeloid commitment .
	manualset3
173203	6	413482	7	NULL	NULL	0	NULL	myeloid commitment	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data also indicate that a coordinated program of lymphoid gene expression involving TdT-CD7-expression and Ig/T beta rearrangements can be activated before myeloid commitment .
	manualset3
173204	1	413483	7	NULL	NULL	0	NULL	 data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data are consistent with the function of LuxS as an important metabolic enzyme but appear not to support the role of AI-2 as a true signal molecule for E. coli W3110 under the investigated conditions .
	manualset3
173205	2	413483	7	NULL	NULL	0	NULL	function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data are consistent with the function of LuxS as an important metabolic enzyme but appear not to support the role of AI-2 as a true signal molecule for E. coli W3110 under the investigated conditions .
	manualset3
173206	3	413483	7	NULL	NULL	0	NULL	LuxS	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data are consistent with the function of LuxS as an important metabolic enzyme but appear not to support the role of AI-2 as a true signal molecule for E. coli W3110 under the investigated conditions .
	manualset3
173207	4	413483	7	NULL	NULL	0	NULL	metabolic enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data are consistent with the function of LuxS as an important metabolic enzyme but appear not to support the role of AI-2 as a true signal molecule for E. coli W3110 under the investigated conditions .
	manualset3
173208	5	413483	7	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data are consistent with the function of LuxS as an important metabolic enzyme but appear not to support the role of AI-2 as a true signal molecule for E. coli W3110 under the investigated conditions .
	manualset3
173209	6	413483	7	NULL	NULL	0	NULL	AI-2	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data are consistent with the function of LuxS as an important metabolic enzyme but appear not to support the role of AI-2 as a true signal molecule for E. coli W3110 under the investigated conditions .
	manualset3
173210	7	413483	7	NULL	NULL	0	NULL	true signal molecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	These data are consistent with the function of LuxS as an important metabolic enzyme but appear not to support the role of AI-2 as a true signal molecule for E. coli W3110 under the investigated conditions .
	manualset3
173211	8	413483	7	NULL	NULL	0	NULL	 E. coli W3110	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These data are consistent with the function of LuxS as an important metabolic enzyme but appear not to support the role of AI-2 as a true signal molecule for E. coli W3110 under the investigated conditions .
	manualset3
173212	9	413483	7	NULL	NULL	0	NULL	investigated conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These data are consistent with the function of LuxS as an important metabolic enzyme but appear not to support the role of AI-2 as a true signal molecule for E. coli W3110 under the investigated conditions .
	manualset3
173213	1	413484	7	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data are discussed in terms of changes and differences in endogenous antidiuretic hormone ( A.D.H. ) release .7 .
	manualset3
173214	2	413484	7	NULL	NULL	NULL	NULL	changes	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data are discussed in terms of changes and differences in endogenous antidiuretic hormone ( A.D.H. ) release .7 .
	manualset3
173215	3	413484	7	NULL	NULL	NULL	NULL	differences	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data are discussed in terms of changes and differences in endogenous antidiuretic hormone ( A.D.H. ) release .7 .
	manualset3
173216	4	413484	7	NULL	NULL	0	NULL	endogenous antidiuretic hormone ( A.D.H. ) release .7 .	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data are discussed in terms of changes and differences in endogenous antidiuretic hormone ( A.D.H. ) release .7 .
	manualset3
173217	1	413485	7	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data can be manipulated and presented in tabular or graphic form on a personal computer and used by hospitals to monitor various drug-use indicators .
	manualset3
173218	2	413485	7	NULL	NULL	0	NULL	tabular or graphic form	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These data can be manipulated and presented in tabular or graphic form on a personal computer and used by hospitals to monitor various drug-use indicators .
	manualset3
173219	3	413485	7	NULL	NULL	NULL	NULL	 personal computer	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data can be manipulated and presented in tabular or graphic form on a personal computer and used by hospitals to monitor various drug-use indicators .
	manualset3
173220	4	413485	7	NULL	NULL	0	NULL	hospitals	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	These data can be manipulated and presented in tabular or graphic form on a personal computer and used by hospitals to monitor various drug-use indicators .
	manualset3
173221	5	413485	7	NULL	NULL	0	NULL	drug-use indicators	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data can be manipulated and presented in tabular or graphic form on a personal computer and used by hospitals to monitor various drug-use indicators .
	manualset3
173222	1	413486	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate an increased microvascular pressure head of O2 at any given point after the initial time delay for Sol versus Per following the onset of contractions that is probably due to faster QO2 dynamics relative to those of VO2 .
	manualset3
173223	2	413486	7	NULL	NULL	NULL	NULL	increased microvascular pressure head	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data demonstrate an increased microvascular pressure head of O2 at any given point after the initial time delay for Sol versus Per following the onset of contractions that is probably due to faster QO2 dynamics relative to those of VO2 .
	manualset3
173224	3	413486	7	NULL	NULL	0	NULL	O2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate an increased microvascular pressure head of O2 at any given point after the initial time delay for Sol versus Per following the onset of contractions that is probably due to faster QO2 dynamics relative to those of VO2 .
	manualset3
173225	4	413486	7	NULL	NULL	0	NULL	point 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate an increased microvascular pressure head of O2 at any given point after the initial time delay for Sol versus Per following the onset of contractions that is probably due to faster QO2 dynamics relative to those of VO2 .
	manualset3
173226	5	413486	7	NULL	NULL	NULL	NULL	initial time delay 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data demonstrate an increased microvascular pressure head of O2 at any given point after the initial time delay for Sol versus Per following the onset of contractions that is probably due to faster QO2 dynamics relative to those of VO2 .
	manualset3
173227	6	413486	7	NULL	NULL	0	NULL	Sol	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate an increased microvascular pressure head of O2 at any given point after the initial time delay for Sol versus Per following the onset of contractions that is probably due to faster QO2 dynamics relative to those of VO2 .
	manualset3
173228	7	413486	7	NULL	NULL	0	NULL	 Per	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate an increased microvascular pressure head of O2 at any given point after the initial time delay for Sol versus Per following the onset of contractions that is probably due to faster QO2 dynamics relative to those of VO2 .
	manualset3
173229	8	413486	7	NULL	NULL	NULL	NULL	onset of contractions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data demonstrate an increased microvascular pressure head of O2 at any given point after the initial time delay for Sol versus Per following the onset of contractions that is probably due to faster QO2 dynamics relative to those of VO2 .
	manualset3
173231	10	413486	7	NULL	NULL	0	NULL	faster QO2 dynamics	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate an increased microvascular pressure head of O2 at any given point after the initial time delay for Sol versus Per following the onset of contractions that is probably due to faster QO2 dynamics relative to those of VO2 .
	manualset3
173232	11	413486	7	NULL	NULL	0	NULL	VO2 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate an increased microvascular pressure head of O2 at any given point after the initial time delay for Sol versus Per following the onset of contractions that is probably due to faster QO2 dynamics relative to those of VO2 .
	manualset3
173233	1	413487	7	NULL	NULL	NULL	NULL	Acute panmyelosis 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Acute panmyelosis with myelofibrosis : clinical , immunophenotypic and cytogenetic study of twelve cases .
	manualset3
173234	2	413487	7	NULL	NULL	0	NULL	 clinical study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute panmyelosis with myelofibrosis : clinical , immunophenotypic and cytogenetic study of twelve cases .
	manualset3
173235	3	413487	7	NULL	NULL	0	NULL	immunophenotypic study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute panmyelosis with myelofibrosis : clinical , immunophenotypic and cytogenetic study of twelve cases .
	manualset3
173236	4	413487	7	NULL	NULL	0	NULL	cytogenetic study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute panmyelosis with myelofibrosis : clinical , immunophenotypic and cytogenetic study of twelve cases .
	manualset3
173237	5	413487	7	NULL	NULL	NULL	NULL	twelve cases	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Acute panmyelosis with myelofibrosis : clinical , immunophenotypic and cytogenetic study of twelve cases .
	manualset3
175212	6	413487	7	NULL	NULL	0	NULL	myelofibrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute panmyelosis with myelofibrosis : clinical , immunophenotypic and cytogenetic study of twelve cases .
	manualset3
173238	1	413488	7	NULL	NULL	0	NULL	 data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate that AP neurons are directly influenced by ORX-A and suggest that ORX-A may exert its effects on the central control of feeding behavior and cardiovascular function through direct actions in AP .
	manualset3
173239	2	413488	7	NULL	NULL	0	NULL	AP neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate that AP neurons are directly influenced by ORX-A and suggest that ORX-A may exert its effects on the central control of feeding behavior and cardiovascular function through direct actions in AP .
	manualset3
173240	3	413488	7	NULL	NULL	0	NULL	ORX-A	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate that AP neurons are directly influenced by ORX-A and suggest that ORX-A may exert its effects on the central control of feeding behavior and cardiovascular function through direct actions in AP .
	manualset3
173241	4	413488	7	NULL	NULL	0	NULL	 ORX-A	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate that AP neurons are directly influenced by ORX-A and suggest that ORX-A may exert its effects on the central control of feeding behavior and cardiovascular function through direct actions in AP .
	manualset3
173242	5	413488	7	NULL	NULL	0	NULL	central control	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate that AP neurons are directly influenced by ORX-A and suggest that ORX-A may exert its effects on the central control of feeding behavior and cardiovascular function through direct actions in AP .
	manualset3
173243	6	413488	7	NULL	NULL	0	NULL	 feeding behavior	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate that AP neurons are directly influenced by ORX-A and suggest that ORX-A may exert its effects on the central control of feeding behavior and cardiovascular function through direct actions in AP .
	manualset3
173244	7	413488	7	NULL	NULL	0	NULL	cardiovascular function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate that AP neurons are directly influenced by ORX-A and suggest that ORX-A may exert its effects on the central control of feeding behavior and cardiovascular function through direct actions in AP .
	manualset3
173245	8	413488	7	NULL	NULL	0	NULL	direct actions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate that AP neurons are directly influenced by ORX-A and suggest that ORX-A may exert its effects on the central control of feeding behavior and cardiovascular function through direct actions in AP .
	manualset3
173246	9	413488	7	NULL	NULL	0	NULL	 AP	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate that AP neurons are directly influenced by ORX-A and suggest that ORX-A may exert its effects on the central control of feeding behavior and cardiovascular function through direct actions in AP .
	manualset3
173247	10	413488	7	NULL	NULL	0	NULL	effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate that AP neurons are directly influenced by ORX-A and suggest that ORX-A may exert its effects on the central control of feeding behavior and cardiovascular function through direct actions in AP .
	manualset3
173248	1	413489	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate that MK-4 is the predominant form of vitamin K in multiple tissues , but there appears to be a tissue-specific regulation for the conversion of PK to MK-4 .
	manualset3
173249	2	413489	7	NULL	NULL	0	NULL	MK-4	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate that MK-4 is the predominant form of vitamin K in multiple tissues , but there appears to be a tissue-specific regulation for the conversion of PK to MK-4 .
	manualset3
173250	3	413489	7	NULL	NULL	0	NULL	predominant form	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate that MK-4 is the predominant form of vitamin K in multiple tissues , but there appears to be a tissue-specific regulation for the conversion of PK to MK-4 .
	manualset3
173251	4	413489	7	NULL	NULL	0	NULL	vitamin K 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate that MK-4 is the predominant form of vitamin K in multiple tissues , but there appears to be a tissue-specific regulation for the conversion of PK to MK-4 .
	manualset3
173252	5	413489	7	NULL	NULL	0	NULL	multiple tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate that MK-4 is the predominant form of vitamin K in multiple tissues , but there appears to be a tissue-specific regulation for the conversion of PK to MK-4 .
	manualset3
173253	6	413489	7	NULL	NULL	0	NULL	tissue-specific regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate that MK-4 is the predominant form of vitamin K in multiple tissues , but there appears to be a tissue-specific regulation for the conversion of PK to MK-4 .
	manualset3
173254	7	413489	7	NULL	NULL	0	NULL	 conversion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate that MK-4 is the predominant form of vitamin K in multiple tissues , but there appears to be a tissue-specific regulation for the conversion of PK to MK-4 .
	manualset3
173255	8	413489	7	NULL	NULL	0	NULL	PK 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate that MK-4 is the predominant form of vitamin K in multiple tissues , but there appears to be a tissue-specific regulation for the conversion of PK to MK-4 .
	manualset3
173256	9	413489	7	NULL	NULL	0	NULL	MK-4 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate that MK-4 is the predominant form of vitamin K in multiple tissues , but there appears to be a tissue-specific regulation for the conversion of PK to MK-4 .
	manualset3
173257	1	413490	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate the occurrence of lipid peroxidation which , however , may not be involved in the observed structure-function changes due to calcium paradox .
	manualset3
173258	2	413490	7	NULL	NULL	0	NULL	 occurrence	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate the occurrence of lipid peroxidation which , however , may not be involved in the observed structure-function changes due to calcium paradox .
	manualset3
173259	3	413490	7	NULL	NULL	0	NULL	lipid peroxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate the occurrence of lipid peroxidation which , however , may not be involved in the observed structure-function changes due to calcium paradox .
	manualset3
173260	4	413490	7	NULL	NULL	0	NULL	structure-function changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate the occurrence of lipid peroxidation which , however , may not be involved in the observed structure-function changes due to calcium paradox .
	manualset3
173261	5	413490	7	NULL	NULL	0	NULL	calcium paradox	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data demonstrate the occurrence of lipid peroxidation which , however , may not be involved in the observed structure-function changes due to calcium paradox .
	manualset3
173262	1	413491	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data have been clearly influenced by the type of surgery .
	manualset3
173263	2	413491	7	NULL	NULL	0	NULL	type	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These data have been clearly influenced by the type of surgery .
	manualset3
173264	3	413491	7	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These data have been clearly influenced by the type of surgery .
	manualset3
173265	1	413492	7	NULL	NULL	0	NULL	 data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data have major implications for the targeting of ST2 as a therapy for allergic airway disorders .
	manualset3
173266	2	413492	7	NULL	NULL	0	NULL	major implications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These data have major implications for the targeting of ST2 as a therapy for allergic airway disorders .
	manualset3
173267	3	413492	7	NULL	NULL	0	NULL	 targeting 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These data have major implications for the targeting of ST2 as a therapy for allergic airway disorders .
	manualset3
173268	4	413492	7	NULL	NULL	0	NULL	ST2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data have major implications for the targeting of ST2 as a therapy for allergic airway disorders .
	manualset3
173269	5	413492	7	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These data have major implications for the targeting of ST2 as a therapy for allergic airway disorders .
	manualset3
173270	6	413492	7	NULL	NULL	NULL	NULL	allergic airway disorders	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data have major implications for the targeting of ST2 as a therapy for allergic airway disorders .
	manualset3
173271	1	413493	7	NULL	NULL	0	NULL	 data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data highlight remarkable photochemical properties for these reaction intermediates , not previously suspected for iron-peroxide species formed in the SOR active site .
	manualset3
173272	2	413493	7	NULL	NULL	0	NULL	photochemical properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data highlight remarkable photochemical properties for these reaction intermediates , not previously suspected for iron-peroxide species formed in the SOR active site .
	manualset3
173273	3	413493	7	NULL	NULL	0	NULL	reaction intermediates	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data highlight remarkable photochemical properties for these reaction intermediates , not previously suspected for iron-peroxide species formed in the SOR active site .
	manualset3
173274	4	413493	7	NULL	NULL	0	NULL	 iron-peroxide species	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data highlight remarkable photochemical properties for these reaction intermediates , not previously suspected for iron-peroxide species formed in the SOR active site .
	manualset3
173275	5	413493	7	NULL	NULL	0	NULL	SOR active site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data highlight remarkable photochemical properties for these reaction intermediates , not previously suspected for iron-peroxide species formed in the SOR active site .
	manualset3
173276	1	413494	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data implicate EAA and particularly NMDA receptors in the RVM in modulating the transmission of opioid pain-inhibitory signals from the PAG .
	manualset3
173277	2	413494	7	NULL	NULL	0	NULL	EAA receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These data implicate EAA and particularly NMDA receptors in the RVM in modulating the transmission of opioid pain-inhibitory signals from the PAG .
	manualset3
173278	3	413494	7	NULL	NULL	0	NULL	NMDA receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These data implicate EAA and particularly NMDA receptors in the RVM in modulating the transmission of opioid pain-inhibitory signals from the PAG .
	manualset3
173279	4	413494	7	NULL	NULL	0	NULL	RVM	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These data implicate EAA and particularly NMDA receptors in the RVM in modulating the transmission of opioid pain-inhibitory signals from the PAG .
	manualset3
173280	5	413494	7	NULL	NULL	0	NULL	 transmission 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data implicate EAA and particularly NMDA receptors in the RVM in modulating the transmission of opioid pain-inhibitory signals from the PAG .
	manualset3
173281	6	413494	7	NULL	NULL	0	NULL	opioid pain-inhibitory signals	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data implicate EAA and particularly NMDA receptors in the RVM in modulating the transmission of opioid pain-inhibitory signals from the PAG .
	manualset3
173282	7	413494	7	NULL	NULL	0	NULL	PAG	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These data implicate EAA and particularly NMDA receptors in the RVM in modulating the transmission of opioid pain-inhibitory signals from the PAG .
	manualset3
173283	1	413495	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that CF is an effector molecule in monocyte-mediated DDCC .
	manualset3
173284	2	413495	7	NULL	NULL	0	NULL	CF	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that CF is an effector molecule in monocyte-mediated DDCC .
	manualset3
173285	3	413495	7	NULL	NULL	0	NULL	effector molecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that CF is an effector molecule in monocyte-mediated DDCC .
	manualset3
173286	4	413495	7	NULL	NULL	0	NULL	monocyte-mediated DDCC	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that CF is an effector molecule in monocyte-mediated DDCC .
	manualset3
173287	1	413496	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that E2-induced mtROS are involved in the regulation of early G1-phase progression .
	manualset3
173288	2	413496	7	NULL	NULL	0	NULL	E2-induced mtROS	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that E2-induced mtROS are involved in the regulation of early G1-phase progression .
	manualset3
173289	3	413496	7	NULL	NULL	0	NULL	regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that E2-induced mtROS are involved in the regulation of early G1-phase progression .
	manualset3
173290	4	413496	7	NULL	NULL	0	NULL	early G1-phase progression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that E2-induced mtROS are involved in the regulation of early G1-phase progression .
	manualset3
173291	1	413497	7	NULL	NULL	0	NULL	Acute renal failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute renal failure was induced by the unilateral clamping of the left renal artery for 60 min , followed by reperfusion and contralateral nephrectomy .
	manualset3
173292	2	413497	7	NULL	NULL	0	NULL	unilateral clamping	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute renal failure was induced by the unilateral clamping of the left renal artery for 60 min , followed by reperfusion and contralateral nephrectomy .
	manualset3
173293	3	413497	7	NULL	NULL	0	NULL	left renal artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute renal failure was induced by the unilateral clamping of the left renal artery for 60 min , followed by reperfusion and contralateral nephrectomy .
	manualset3
173294	4	413497	7	NULL	NULL	0	NULL	60 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute renal failure was induced by the unilateral clamping of the left renal artery for 60 min , followed by reperfusion and contralateral nephrectomy .
	manualset3
173295	5	413497	7	NULL	NULL	NULL	NULL	reperfusion	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Acute renal failure was induced by the unilateral clamping of the left renal artery for 60 min , followed by reperfusion and contralateral nephrectomy .
	manualset3
173296	6	413497	7	NULL	NULL	NULL	NULL	contralateral nephrectomy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Acute renal failure was induced by the unilateral clamping of the left renal artery for 60 min , followed by reperfusion and contralateral nephrectomy .
	manualset3
173297	1	413498	7	NULL	NULL	0	NULL	 data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that laminin-induced activation of PLD and consequent generation of phosphatidic acid are involved in a signal propagation pathway leading to induction of MMP-2 and enhanced invasiveness of metastatic tumor cells .
	manualset3
173298	2	413498	7	NULL	NULL	0	NULL	laminin-induced activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that laminin-induced activation of PLD and consequent generation of phosphatidic acid are involved in a signal propagation pathway leading to induction of MMP-2 and enhanced invasiveness of metastatic tumor cells .
	manualset3
173299	3	413498	7	NULL	NULL	0	NULL	PLD	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that laminin-induced activation of PLD and consequent generation of phosphatidic acid are involved in a signal propagation pathway leading to induction of MMP-2 and enhanced invasiveness of metastatic tumor cells .
	manualset3
173300	4	413498	7	NULL	NULL	0	NULL	generation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that laminin-induced activation of PLD and consequent generation of phosphatidic acid are involved in a signal propagation pathway leading to induction of MMP-2 and enhanced invasiveness of metastatic tumor cells .
	manualset3
173301	5	413498	7	NULL	NULL	0	NULL	phosphatidic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that laminin-induced activation of PLD and consequent generation of phosphatidic acid are involved in a signal propagation pathway leading to induction of MMP-2 and enhanced invasiveness of metastatic tumor cells .
	manualset3
173302	6	413498	7	NULL	NULL	0	NULL	signal propagation pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that laminin-induced activation of PLD and consequent generation of phosphatidic acid are involved in a signal propagation pathway leading to induction of MMP-2 and enhanced invasiveness of metastatic tumor cells .
	manualset3
173303	7	413498	7	NULL	NULL	0	NULL	induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that laminin-induced activation of PLD and consequent generation of phosphatidic acid are involved in a signal propagation pathway leading to induction of MMP-2 and enhanced invasiveness of metastatic tumor cells .
	manualset3
173304	8	413498	7	NULL	NULL	0	NULL	MMP-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that laminin-induced activation of PLD and consequent generation of phosphatidic acid are involved in a signal propagation pathway leading to induction of MMP-2 and enhanced invasiveness of metastatic tumor cells .
	manualset3
173305	9	413498	7	NULL	NULL	0	NULL	enhanced invasiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that laminin-induced activation of PLD and consequent generation of phosphatidic acid are involved in a signal propagation pathway leading to induction of MMP-2 and enhanced invasiveness of metastatic tumor cells .
	manualset3
173306	10	413498	7	NULL	NULL	0	NULL	metastatic tumor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that laminin-induced activation of PLD and consequent generation of phosphatidic acid are involved in a signal propagation pathway leading to induction of MMP-2 and enhanced invasiveness of metastatic tumor cells .
	manualset3
173334	1	413499	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that neurite outgrowth activity of peptide-alginate matrices is peptide specific and the activity is dependent on the amount of alginate .
	manualset3
173336	2	413499	7	NULL	NULL	NULL	NULL	neurite outgrowth activity 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data indicate that neurite outgrowth activity of peptide-alginate matrices is peptide specific and the activity is dependent on the amount of alginate .
	manualset3
173337	3	413499	7	NULL	NULL	0	NULL	peptide-alginate matrices 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that neurite outgrowth activity of peptide-alginate matrices is peptide specific and the activity is dependent on the amount of alginate .
	manualset3
173340	5	413499	7	NULL	NULL	0	NULL	activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that neurite outgrowth activity of peptide-alginate matrices is peptide specific and the activity is dependent on the amount of alginate .
	manualset3
173341	6	413499	7	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that neurite outgrowth activity of peptide-alginate matrices is peptide specific and the activity is dependent on the amount of alginate .
	manualset3
173344	7	413499	7	NULL	NULL	0	NULL	alginate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that neurite outgrowth activity of peptide-alginate matrices is peptide specific and the activity is dependent on the amount of alginate .
	manualset3
173346	1	413500	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that platelets , through the release of purine nucleotides , enhance superoxide generation by neutrophils , thus increasing the cytotoxic potential of these cells .
	manualset3
173347	2	413500	7	NULL	NULL	0	NULL	platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that platelets , through the release of purine nucleotides , enhance superoxide generation by neutrophils , thus increasing the cytotoxic potential of these cells .
	manualset3
173348	3	413500	7	NULL	NULL	0	NULL	release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that platelets , through the release of purine nucleotides , enhance superoxide generation by neutrophils , thus increasing the cytotoxic potential of these cells .
	manualset3
173349	4	413500	7	NULL	NULL	0	NULL	purine nucleotides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that platelets , through the release of purine nucleotides , enhance superoxide generation by neutrophils , thus increasing the cytotoxic potential of these cells .
	manualset3
173350	5	413500	7	NULL	NULL	NULL	NULL	superoxide generation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data indicate that platelets , through the release of purine nucleotides , enhance superoxide generation by neutrophils , thus increasing the cytotoxic potential of these cells .
	manualset3
173351	6	413500	7	NULL	NULL	0	NULL	neutrophils	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that platelets , through the release of purine nucleotides , enhance superoxide generation by neutrophils , thus increasing the cytotoxic potential of these cells .
	manualset3
173352	7	413500	7	NULL	NULL	0	NULL	cytotoxic potential	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that platelets , through the release of purine nucleotides , enhance superoxide generation by neutrophils , thus increasing the cytotoxic potential of these cells .
	manualset3
173353	8	413500	7	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that platelets , through the release of purine nucleotides , enhance superoxide generation by neutrophils , thus increasing the cytotoxic potential of these cells .
	manualset3
173354	1	413501	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that the beta 2-receptor agonistic and anti-permeability actions of terbutaline are found solely in the levorotatory enantiomer .
	manualset3
173359	2	413501	7	NULL	NULL	0	NULL	beta 2-receptor agonistic actions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that the beta 2-receptor agonistic and anti-permeability actions of terbutaline are found solely in the levorotatory enantiomer .
	manualset3
173361	3	413501	7	NULL	NULL	NULL	NULL	anti-permeability actions	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data indicate that the beta 2-receptor agonistic and anti-permeability actions of terbutaline are found solely in the levorotatory enantiomer .
	manualset3
173362	4	413501	7	NULL	NULL	0	NULL	terbutaline	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that the beta 2-receptor agonistic and anti-permeability actions of terbutaline are found solely in the levorotatory enantiomer .
	manualset3
173363	5	413501	7	NULL	NULL	0	NULL	levorotatory enantiomer	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that the beta 2-receptor agonistic and anti-permeability actions of terbutaline are found solely in the levorotatory enantiomer .
	manualset3
173408	1	413502	7	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that the hormone-sensitive pool of hepatocyte phosphoinositides can be labeled by both in vitro and in vivo procedures .
	manualset3
173409	2	413502	7	NULL	NULL	0	NULL	hormone-sensitive pool 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that the hormone-sensitive pool of hepatocyte phosphoinositides can be labeled by both in vitro and in vivo procedures .
	manualset3
173410	3	413502	7	NULL	NULL	NULL	NULL	hepatocyte phosphoinositides	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data indicate that the hormone-sensitive pool of hepatocyte phosphoinositides can be labeled by both in vitro and in vivo procedures .
	manualset3
173411	4	413502	7	NULL	NULL	0	NULL	 in vitro procedures	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that the hormone-sensitive pool of hepatocyte phosphoinositides can be labeled by both in vitro and in vivo procedures .
	manualset3
173412	5	413502	7	NULL	NULL	0	NULL	in vivo procedures	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that the hormone-sensitive pool of hepatocyte phosphoinositides can be labeled by both in vitro and in vivo procedures .
	manualset3
173416	1	413503	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data offer the prospect of designing vectors that will confer resistance to entire regimens of chemotherapy rather than just to individual components of such drug cocktails , thereby substantially increasing the efficacy of therapy .
	manualset3
173417	2	413503	7	NULL	NULL	0	NULL	prospect 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data offer the prospect of designing vectors that will confer resistance to entire regimens of chemotherapy rather than just to individual components of such drug cocktails , thereby substantially increasing the efficacy of therapy .
	manualset3
173418	3	413503	7	NULL	NULL	0	NULL	designing vectors	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data offer the prospect of designing vectors that will confer resistance to entire regimens of chemotherapy rather than just to individual components of such drug cocktails , thereby substantially increasing the efficacy of therapy .
	manualset3
173419	4	413503	7	NULL	NULL	NULL	NULL	resistance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data offer the prospect of designing vectors that will confer resistance to entire regimens of chemotherapy rather than just to individual components of such drug cocktails , thereby substantially increasing the efficacy of therapy .
	manualset3
173420	5	413503	7	NULL	NULL	0	NULL	entire regimens	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These data offer the prospect of designing vectors that will confer resistance to entire regimens of chemotherapy rather than just to individual components of such drug cocktails , thereby substantially increasing the efficacy of therapy .
	manualset3
173421	6	413503	7	NULL	NULL	0	NULL	chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These data offer the prospect of designing vectors that will confer resistance to entire regimens of chemotherapy rather than just to individual components of such drug cocktails , thereby substantially increasing the efficacy of therapy .
	manualset3
173422	7	413503	7	NULL	NULL	NULL	NULL	individual components	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data offer the prospect of designing vectors that will confer resistance to entire regimens of chemotherapy rather than just to individual components of such drug cocktails , thereby substantially increasing the efficacy of therapy .
	manualset3
173423	8	413503	7	NULL	NULL	0	NULL	drug cocktails	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These data offer the prospect of designing vectors that will confer resistance to entire regimens of chemotherapy rather than just to individual components of such drug cocktails , thereby substantially increasing the efficacy of therapy .
	manualset3
173424	9	413503	7	NULL	NULL	0	NULL	efficacy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These data offer the prospect of designing vectors that will confer resistance to entire regimens of chemotherapy rather than just to individual components of such drug cocktails , thereby substantially increasing the efficacy of therapy .
	manualset3
173425	10	413503	7	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These data offer the prospect of designing vectors that will confer resistance to entire regimens of chemotherapy rather than just to individual components of such drug cocktails , thereby substantially increasing the efficacy of therapy .
	manualset3
173426	1	413504	7	NULL	NULL	0	NULL	 data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data provide the first direct evidence that activation of intracellular CaMKII signaling in the PPT promotes W and suppresses sleep .
	manualset3
173427	2	413504	7	NULL	NULL	0	NULL	direct evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These data provide the first direct evidence that activation of intracellular CaMKII signaling in the PPT promotes W and suppresses sleep .
	manualset3
173428	3	413504	7	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data provide the first direct evidence that activation of intracellular CaMKII signaling in the PPT promotes W and suppresses sleep .
	manualset3
173429	4	413504	7	NULL	NULL	0	NULL	intracellular CaMKII signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data provide the first direct evidence that activation of intracellular CaMKII signaling in the PPT promotes W and suppresses sleep .
	manualset3
173430	5	413504	7	NULL	NULL	0	NULL	PPT	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data provide the first direct evidence that activation of intracellular CaMKII signaling in the PPT promotes W and suppresses sleep .
	manualset3
173431	6	413504	7	NULL	NULL	0	NULL	W	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data provide the first direct evidence that activation of intracellular CaMKII signaling in the PPT promotes W and suppresses sleep .
	manualset3
173432	7	413504	7	NULL	NULL	0	NULL	sleep	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data provide the first direct evidence that activation of intracellular CaMKII signaling in the PPT promotes W and suppresses sleep .
	manualset3
173433	1	413505	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data provided strong evidence that approximately 65 % of threonine oxidation occurs through the glycine-independent threonine dehydratase pathway .
	manualset3
173434	2	413505	7	NULL	NULL	0	NULL	strong evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These data provided strong evidence that approximately 65 % of threonine oxidation occurs through the glycine-independent threonine dehydratase pathway .
	manualset3
173435	3	413505	7	NULL	NULL	0	NULL	65 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These data provided strong evidence that approximately 65 % of threonine oxidation occurs through the glycine-independent threonine dehydratase pathway .
	manualset3
173436	4	413505	7	NULL	NULL	0	NULL	threonine oxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data provided strong evidence that approximately 65 % of threonine oxidation occurs through the glycine-independent threonine dehydratase pathway .
	manualset3
173437	5	413505	7	NULL	NULL	0	NULL	glycine-independent threonine dehydratase pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data provided strong evidence that approximately 65 % of threonine oxidation occurs through the glycine-independent threonine dehydratase pathway .
	manualset3
173438	1	413506	7	NULL	NULL	0	NULL	Acute respiratory distress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute respiratory distress due to malignant schwannoma .
	manualset3
173439	2	413506	7	NULL	NULL	0	NULL	malignant schwannoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute respiratory distress due to malignant schwannoma .
	manualset3
173440	1	413507	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data reflect a high standard of care of patients dying of cancer and other chronic diseases in an acute hospital environment , but do not demonstrate a difference between the two models of service delivery of specialist palliative care .
	manualset3
173441	2	413507	7	NULL	NULL	0	NULL	 high standard 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data reflect a high standard of care of patients dying of cancer and other chronic diseases in an acute hospital environment , but do not demonstrate a difference between the two models of service delivery of specialist palliative care .
	manualset3
173442	3	413507	7	NULL	NULL	0	NULL	care 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	These data reflect a high standard of care of patients dying of cancer and other chronic diseases in an acute hospital environment , but do not demonstrate a difference between the two models of service delivery of specialist palliative care .
	manualset3
173443	4	413507	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These data reflect a high standard of care of patients dying of cancer and other chronic diseases in an acute hospital environment , but do not demonstrate a difference between the two models of service delivery of specialist palliative care .
	manualset3
173444	5	413507	7	NULL	NULL	0	NULL	cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These data reflect a high standard of care of patients dying of cancer and other chronic diseases in an acute hospital environment , but do not demonstrate a difference between the two models of service delivery of specialist palliative care .
	manualset3
173445	6	413507	7	NULL	NULL	0	NULL	chronic diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These data reflect a high standard of care of patients dying of cancer and other chronic diseases in an acute hospital environment , but do not demonstrate a difference between the two models of service delivery of specialist palliative care .
	manualset3
173446	7	413507	7	NULL	NULL	0	NULL	acute hospital environment	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	These data reflect a high standard of care of patients dying of cancer and other chronic diseases in an acute hospital environment , but do not demonstrate a difference between the two models of service delivery of specialist palliative care .
	manualset3
173447	8	413507	7	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These data reflect a high standard of care of patients dying of cancer and other chronic diseases in an acute hospital environment , but do not demonstrate a difference between the two models of service delivery of specialist palliative care .
	manualset3
173448	9	413507	7	NULL	NULL	0	NULL	 two models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These data reflect a high standard of care of patients dying of cancer and other chronic diseases in an acute hospital environment , but do not demonstrate a difference between the two models of service delivery of specialist palliative care .
	manualset3
173449	10	413507	7	NULL	NULL	0	NULL	service delivery	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	These data reflect a high standard of care of patients dying of cancer and other chronic diseases in an acute hospital environment , but do not demonstrate a difference between the two models of service delivery of specialist palliative care .
	manualset3
173450	11	413507	7	NULL	NULL	0	NULL	specialist palliative care	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	These data reflect a high standard of care of patients dying of cancer and other chronic diseases in an acute hospital environment , but do not demonstrate a difference between the two models of service delivery of specialist palliative care .
	manualset3
173451	1	413508	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show that children with sickle cell anemia are not deficient in essential fatty acids , but that the fatty acid elongation and desaturation pathway is somehow disturbed in this disease .
	manualset3
173452	2	413508	7	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show that children with sickle cell anemia are not deficient in essential fatty acids , but that the fatty acid elongation and desaturation pathway is somehow disturbed in this disease .
	manualset3
173453	3	413508	7	NULL	NULL	0	NULL	sickle cell anemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show that children with sickle cell anemia are not deficient in essential fatty acids , but that the fatty acid elongation and desaturation pathway is somehow disturbed in this disease .
	manualset3
173454	4	413508	7	NULL	NULL	0	NULL	deficient 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show that children with sickle cell anemia are not deficient in essential fatty acids , but that the fatty acid elongation and desaturation pathway is somehow disturbed in this disease .
	manualset3
173455	5	413508	7	NULL	NULL	0	NULL	essential fatty acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show that children with sickle cell anemia are not deficient in essential fatty acids , but that the fatty acid elongation and desaturation pathway is somehow disturbed in this disease .
	manualset3
173456	6	413508	7	NULL	NULL	0	NULL	fatty acid elongation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show that children with sickle cell anemia are not deficient in essential fatty acids , but that the fatty acid elongation and desaturation pathway is somehow disturbed in this disease .
	manualset3
173457	7	413508	7	NULL	NULL	0	NULL	desaturation pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show that children with sickle cell anemia are not deficient in essential fatty acids , but that the fatty acid elongation and desaturation pathway is somehow disturbed in this disease .
	manualset3
173458	8	413508	7	NULL	NULL	0	NULL	disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show that children with sickle cell anemia are not deficient in essential fatty acids , but that the fatty acid elongation and desaturation pathway is somehow disturbed in this disease .
	manualset3
173459	1	413509	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show that electrolyte solutions behave like a supercooled liquid approaching a glass transition in which rotational and translational molecular motions are decoupled .
	manualset3
173460	2	413509	7	NULL	NULL	0	NULL	electrolyte solutions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show that electrolyte solutions behave like a supercooled liquid approaching a glass transition in which rotational and translational molecular motions are decoupled .
	manualset3
173461	3	413509	7	NULL	NULL	0	NULL	supercooled liquid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show that electrolyte solutions behave like a supercooled liquid approaching a glass transition in which rotational and translational molecular motions are decoupled .
	manualset3
173462	4	413509	7	NULL	NULL	0	NULL	glass transition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show that electrolyte solutions behave like a supercooled liquid approaching a glass transition in which rotational and translational molecular motions are decoupled .
	manualset3
173463	5	413509	7	NULL	NULL	NULL	NULL	rotational molecular motions	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data show that electrolyte solutions behave like a supercooled liquid approaching a glass transition in which rotational and translational molecular motions are decoupled .
	manualset3
173464	6	413509	7	NULL	NULL	NULL	NULL	translational molecular motions	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data show that electrolyte solutions behave like a supercooled liquid approaching a glass transition in which rotational and translational molecular motions are decoupled .
	manualset3
173465	1	413510	7	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show that peroxynitrite stimulates cyclic GMP synthesis , inferring production of low yields of nitric oxide or associated derivatives .
	manualset3
173466	2	413510	7	NULL	NULL	0	NULL	peroxynitrite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show that peroxynitrite stimulates cyclic GMP synthesis , inferring production of low yields of nitric oxide or associated derivatives .
	manualset3
173467	3	413510	7	NULL	NULL	0	NULL	cyclic GMP synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show that peroxynitrite stimulates cyclic GMP synthesis , inferring production of low yields of nitric oxide or associated derivatives .
	manualset3
173468	4	413510	7	NULL	NULL	0	NULL	 production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show that peroxynitrite stimulates cyclic GMP synthesis , inferring production of low yields of nitric oxide or associated derivatives .
	manualset3
173469	5	413510	7	NULL	NULL	0	NULL	low yields	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show that peroxynitrite stimulates cyclic GMP synthesis , inferring production of low yields of nitric oxide or associated derivatives .
	manualset3
173470	6	413510	7	NULL	NULL	0	NULL	nitric oxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show that peroxynitrite stimulates cyclic GMP synthesis , inferring production of low yields of nitric oxide or associated derivatives .
	manualset3
173471	7	413510	7	NULL	NULL	0	NULL	associated derivatives	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show that peroxynitrite stimulates cyclic GMP synthesis , inferring production of low yields of nitric oxide or associated derivatives .
	manualset3
173472	1	413511	7	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show that the blockade of TGF-beta2 within this tumor reduces tumor growth and raises the possibility that TGF-beta2 antisense ODNs may be useful as a therapy for this disease .
	manualset3
173473	2	413511	7	NULL	NULL	0	NULL	blockade	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show that the blockade of TGF-beta2 within this tumor reduces tumor growth and raises the possibility that TGF-beta2 antisense ODNs may be useful as a therapy for this disease .
	manualset3
173474	3	413511	7	NULL	NULL	0	NULL	TGF-beta2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show that the blockade of TGF-beta2 within this tumor reduces tumor growth and raises the possibility that TGF-beta2 antisense ODNs may be useful as a therapy for this disease .
	manualset3
173475	4	413511	7	NULL	NULL	0	NULL	 tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show that the blockade of TGF-beta2 within this tumor reduces tumor growth and raises the possibility that TGF-beta2 antisense ODNs may be useful as a therapy for this disease .
	manualset3
173476	5	413511	7	NULL	NULL	0	NULL	 tumor growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show that the blockade of TGF-beta2 within this tumor reduces tumor growth and raises the possibility that TGF-beta2 antisense ODNs may be useful as a therapy for this disease .
	manualset3
173477	6	413511	7	NULL	NULL	0	NULL	possibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show that the blockade of TGF-beta2 within this tumor reduces tumor growth and raises the possibility that TGF-beta2 antisense ODNs may be useful as a therapy for this disease .
	manualset3
173478	7	413511	7	NULL	NULL	0	NULL	TGF-beta2 antisense ODNs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show that the blockade of TGF-beta2 within this tumor reduces tumor growth and raises the possibility that TGF-beta2 antisense ODNs may be useful as a therapy for this disease .
	manualset3
173479	8	413511	7	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show that the blockade of TGF-beta2 within this tumor reduces tumor growth and raises the possibility that TGF-beta2 antisense ODNs may be useful as a therapy for this disease .
	manualset3
173480	9	413511	7	NULL	NULL	0	NULL	disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show that the blockade of TGF-beta2 within this tumor reduces tumor growth and raises the possibility that TGF-beta2 antisense ODNs may be useful as a therapy for this disease .
	manualset3
173481	1	413512	7	NULL	NULL	0	NULL	 data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data strongly suggest a postcentral origin of the P22 SEP component in Brodmann area 1 and render a major precentral contribution to the earliest stages of processing from the primary motor cortex less likely .
	manualset3
173482	2	413512	7	NULL	NULL	0	NULL	postcentral origin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These data strongly suggest a postcentral origin of the P22 SEP component in Brodmann area 1 and render a major precentral contribution to the earliest stages of processing from the primary motor cortex less likely .
	manualset3
173483	3	413512	7	NULL	NULL	0	NULL	P22 SEP component	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These data strongly suggest a postcentral origin of the P22 SEP component in Brodmann area 1 and render a major precentral contribution to the earliest stages of processing from the primary motor cortex less likely .
	manualset3
173484	4	413512	7	NULL	NULL	0	NULL	Brodmann area 1 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These data strongly suggest a postcentral origin of the P22 SEP component in Brodmann area 1 and render a major precentral contribution to the earliest stages of processing from the primary motor cortex less likely .
	manualset3
173485	5	413512	7	NULL	NULL	NULL	NULL	precentral contribution	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data strongly suggest a postcentral origin of the P22 SEP component in Brodmann area 1 and render a major precentral contribution to the earliest stages of processing from the primary motor cortex less likely .
	manualset3
173486	6	413512	7	NULL	NULL	0	NULL	earliest stages	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	These data strongly suggest a postcentral origin of the P22 SEP component in Brodmann area 1 and render a major precentral contribution to the earliest stages of processing from the primary motor cortex less likely .
	manualset3
173487	7	413512	7	NULL	NULL	0	NULL	primary motor cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These data strongly suggest a postcentral origin of the P22 SEP component in Brodmann area 1 and render a major precentral contribution to the earliest stages of processing from the primary motor cortex less likely .
	manualset3
173488	1	413513	7	NULL	NULL	0	NULL	 data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data strongly suggest that the permissive effect of glucocorticoids towards lipolysis `` in vivo '' results at least in part from a glucocorticoid-receptor mediated action of these hormones on the fat cell membranous components involved in the beta-adrenergic control of lipolysis .
	manualset3
173489	2	413513	7	NULL	NULL	0	NULL	permissive effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data strongly suggest that the permissive effect of glucocorticoids towards lipolysis `` in vivo '' results at least in part from a glucocorticoid-receptor mediated action of these hormones on the fat cell membranous components involved in the beta-adrenergic control of lipolysis .
	manualset3
173490	3	413513	7	NULL	NULL	0	NULL	glucocorticoids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data strongly suggest that the permissive effect of glucocorticoids towards lipolysis `` in vivo '' results at least in part from a glucocorticoid-receptor mediated action of these hormones on the fat cell membranous components involved in the beta-adrenergic control of lipolysis .
	manualset3
173491	4	413513	7	NULL	NULL	0	NULL	lipolysis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data strongly suggest that the permissive effect of glucocorticoids towards lipolysis `` in vivo '' results at least in part from a glucocorticoid-receptor mediated action of these hormones on the fat cell membranous components involved in the beta-adrenergic control of lipolysis .
	manualset3
173492	5	413513	7	NULL	NULL	0	NULL	glucocorticoid-receptor mediated action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data strongly suggest that the permissive effect of glucocorticoids towards lipolysis `` in vivo '' results at least in part from a glucocorticoid-receptor mediated action of these hormones on the fat cell membranous components involved in the beta-adrenergic control of lipolysis .
	manualset3
173493	6	413513	7	NULL	NULL	0	NULL	hormones 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data strongly suggest that the permissive effect of glucocorticoids towards lipolysis `` in vivo '' results at least in part from a glucocorticoid-receptor mediated action of these hormones on the fat cell membranous components involved in the beta-adrenergic control of lipolysis .
	manualset3
173494	7	413513	7	NULL	NULL	0	NULL	fat cell membranous components	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data strongly suggest that the permissive effect of glucocorticoids towards lipolysis `` in vivo '' results at least in part from a glucocorticoid-receptor mediated action of these hormones on the fat cell membranous components involved in the beta-adrenergic control of lipolysis .
	manualset3
173495	8	413513	7	NULL	NULL	0	NULL	beta-adrenergic control	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data strongly suggest that the permissive effect of glucocorticoids towards lipolysis `` in vivo '' results at least in part from a glucocorticoid-receptor mediated action of these hormones on the fat cell membranous components involved in the beta-adrenergic control of lipolysis .
	manualset3
173496	9	413513	7	NULL	NULL	0	NULL	lipolysis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data strongly suggest that the permissive effect of glucocorticoids towards lipolysis `` in vivo '' results at least in part from a glucocorticoid-receptor mediated action of these hormones on the fat cell membranous components involved in the beta-adrenergic control of lipolysis .
	manualset3
173497	1	413514	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest a dichotomy between CD4 ( + ) regulatory T cells positive for the transcription factor Foxp3 and T ( H ) -17 cells : TGF-beta induces Foxp3 and generates induced regulatory T cells , whereas IL-6 inhibits TGF-beta-driven Foxp3 expression and together with TGF-beta induces T ( H ) -17 cells .
	manualset3
173498	2	413514	7	NULL	NULL	0	NULL	dichotomy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest a dichotomy between CD4 ( + ) regulatory T cells positive for the transcription factor Foxp3 and T ( H ) -17 cells : TGF-beta induces Foxp3 and generates induced regulatory T cells , whereas IL-6 inhibits TGF-beta-driven Foxp3 expression and together with TGF-beta induces T ( H ) -17 cells .
	manualset3
173499	3	413514	7	NULL	NULL	0	NULL	CD4 ( + ) regulatory T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest a dichotomy between CD4 ( + ) regulatory T cells positive for the transcription factor Foxp3 and T ( H ) -17 cells : TGF-beta induces Foxp3 and generates induced regulatory T cells , whereas IL-6 inhibits TGF-beta-driven Foxp3 expression and together with TGF-beta induces T ( H ) -17 cells .
	manualset3
173500	4	413514	7	NULL	NULL	0	NULL	transcription factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest a dichotomy between CD4 ( + ) regulatory T cells positive for the transcription factor Foxp3 and T ( H ) -17 cells : TGF-beta induces Foxp3 and generates induced regulatory T cells , whereas IL-6 inhibits TGF-beta-driven Foxp3 expression and together with TGF-beta induces T ( H ) -17 cells .
	manualset3
173501	5	413514	7	NULL	NULL	0	NULL	Foxp3 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest a dichotomy between CD4 ( + ) regulatory T cells positive for the transcription factor Foxp3 and T ( H ) -17 cells : TGF-beta induces Foxp3 and generates induced regulatory T cells , whereas IL-6 inhibits TGF-beta-driven Foxp3 expression and together with TGF-beta induces T ( H ) -17 cells .
	manualset3
173502	6	413514	7	NULL	NULL	0	NULL	T ( H ) -17 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest a dichotomy between CD4 ( + ) regulatory T cells positive for the transcription factor Foxp3 and T ( H ) -17 cells : TGF-beta induces Foxp3 and generates induced regulatory T cells , whereas IL-6 inhibits TGF-beta-driven Foxp3 expression and together with TGF-beta induces T ( H ) -17 cells .
	manualset3
173503	7	413514	7	NULL	NULL	0	NULL	TGF-beta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest a dichotomy between CD4 ( + ) regulatory T cells positive for the transcription factor Foxp3 and T ( H ) -17 cells : TGF-beta induces Foxp3 and generates induced regulatory T cells , whereas IL-6 inhibits TGF-beta-driven Foxp3 expression and together with TGF-beta induces T ( H ) -17 cells .
	manualset3
173504	8	413514	7	NULL	NULL	0	NULL	 Foxp3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest a dichotomy between CD4 ( + ) regulatory T cells positive for the transcription factor Foxp3 and T ( H ) -17 cells : TGF-beta induces Foxp3 and generates induced regulatory T cells , whereas IL-6 inhibits TGF-beta-driven Foxp3 expression and together with TGF-beta induces T ( H ) -17 cells .
	manualset3
173505	9	413514	7	NULL	NULL	0	NULL	regulatory T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest a dichotomy between CD4 ( + ) regulatory T cells positive for the transcription factor Foxp3 and T ( H ) -17 cells : TGF-beta induces Foxp3 and generates induced regulatory T cells , whereas IL-6 inhibits TGF-beta-driven Foxp3 expression and together with TGF-beta induces T ( H ) -17 cells .
	manualset3
173506	10	413514	7	NULL	NULL	0	NULL	IL-6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest a dichotomy between CD4 ( + ) regulatory T cells positive for the transcription factor Foxp3 and T ( H ) -17 cells : TGF-beta induces Foxp3 and generates induced regulatory T cells , whereas IL-6 inhibits TGF-beta-driven Foxp3 expression and together with TGF-beta induces T ( H ) -17 cells .
	manualset3
173507	11	413514	7	NULL	NULL	0	NULL	TGF-beta-driven Foxp3 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest a dichotomy between CD4 ( + ) regulatory T cells positive for the transcription factor Foxp3 and T ( H ) -17 cells : TGF-beta induces Foxp3 and generates induced regulatory T cells , whereas IL-6 inhibits TGF-beta-driven Foxp3 expression and together with TGF-beta induces T ( H ) -17 cells .
	manualset3
173508	12	413514	7	NULL	NULL	0	NULL	 TGF-beta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest a dichotomy between CD4 ( + ) regulatory T cells positive for the transcription factor Foxp3 and T ( H ) -17 cells : TGF-beta induces Foxp3 and generates induced regulatory T cells , whereas IL-6 inhibits TGF-beta-driven Foxp3 expression and together with TGF-beta induces T ( H ) -17 cells .
	manualset3
173509	13	413514	7	NULL	NULL	0	NULL	T ( H ) -17 cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest a dichotomy between CD4 ( + ) regulatory T cells positive for the transcription factor Foxp3 and T ( H ) -17 cells : TGF-beta induces Foxp3 and generates induced regulatory T cells , whereas IL-6 inhibits TGF-beta-driven Foxp3 expression and together with TGF-beta induces T ( H ) -17 cells .
	manualset3
173510	1	413515	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest possible short-term strategies for transfer of ASA into the CNS via transduced autologous cells while long-term strategies , related to autologous transduced bone marrow transplant , take effect in patients .
	manualset3
173511	2	413515	7	NULL	NULL	0	NULL	short-term strategies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest possible short-term strategies for transfer of ASA into the CNS via transduced autologous cells while long-term strategies , related to autologous transduced bone marrow transplant , take effect in patients .
	manualset3
173512	3	413515	7	NULL	NULL	0	NULL	 transfer	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest possible short-term strategies for transfer of ASA into the CNS via transduced autologous cells while long-term strategies , related to autologous transduced bone marrow transplant , take effect in patients .
	manualset3
173513	4	413515	7	NULL	NULL	0	NULL	ASA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest possible short-term strategies for transfer of ASA into the CNS via transduced autologous cells while long-term strategies , related to autologous transduced bone marrow transplant , take effect in patients .
	manualset3
173514	5	413515	7	NULL	NULL	0	NULL	CNS	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest possible short-term strategies for transfer of ASA into the CNS via transduced autologous cells while long-term strategies , related to autologous transduced bone marrow transplant , take effect in patients .
	manualset3
173515	6	413515	7	NULL	NULL	0	NULL	transduced autologous cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest possible short-term strategies for transfer of ASA into the CNS via transduced autologous cells while long-term strategies , related to autologous transduced bone marrow transplant , take effect in patients .
	manualset3
173516	7	413515	7	NULL	NULL	0	NULL	long-term strategies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest possible short-term strategies for transfer of ASA into the CNS via transduced autologous cells while long-term strategies , related to autologous transduced bone marrow transplant , take effect in patients .
	manualset3
173517	8	413515	7	NULL	NULL	NULL	NULL	autologous transduced bone marrow transplant	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data suggest possible short-term strategies for transfer of ASA into the CNS via transduced autologous cells while long-term strategies , related to autologous transduced bone marrow transplant , take effect in patients .
	manualset3
173518	9	413515	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest possible short-term strategies for transfer of ASA into the CNS via transduced autologous cells while long-term strategies , related to autologous transduced bone marrow transplant , take effect in patients .
	manualset3
175275	10	413515	7	NULL	NULL	0	NULL	effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest possible short-term strategies for transfer of ASA into the CNS via transduced autologous cells while long-term strategies , related to autologous transduced bone marrow transplant , take effect in patients .
	manualset3
173519	1	413516	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that , while monoamines in the brain are involved in the behavioral effects of enkephalins , the precise sites and/or mechanisms of enkephalins may differ .
	manualset3
173520	2	413516	7	NULL	NULL	0	NULL	monoamines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that , while monoamines in the brain are involved in the behavioral effects of enkephalins , the precise sites and/or mechanisms of enkephalins may differ .
	manualset3
173521	3	413516	7	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that , while monoamines in the brain are involved in the behavioral effects of enkephalins , the precise sites and/or mechanisms of enkephalins may differ .
	manualset3
173522	4	413516	7	NULL	NULL	0	NULL	behavioral effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that , while monoamines in the brain are involved in the behavioral effects of enkephalins , the precise sites and/or mechanisms of enkephalins may differ .
	manualset3
173523	5	413516	7	NULL	NULL	0	NULL	enkephalins	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that , while monoamines in the brain are involved in the behavioral effects of enkephalins , the precise sites and/or mechanisms of enkephalins may differ .
	manualset3
173524	6	413516	7	NULL	NULL	0	NULL	mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that , while monoamines in the brain are involved in the behavioral effects of enkephalins , the precise sites and/or mechanisms of enkephalins may differ .
	manualset3
173525	7	413516	7	NULL	NULL	0	NULL	enkephalins	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that , while monoamines in the brain are involved in the behavioral effects of enkephalins , the precise sites and/or mechanisms of enkephalins may differ .
	manualset3
173526	8	413516	7	NULL	NULL	0	NULL	precise sites	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that , while monoamines in the brain are involved in the behavioral effects of enkephalins , the precise sites and/or mechanisms of enkephalins may differ .
	manualset3
173527	1	413517	7	NULL	NULL	0	NULL	 data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that EC and CGA have no effect on apoptosis and enhance the intrinsic cellular tolerance against oxidative insults either by activating survival/proliferation pathways or by increasing antioxidant potential in HepG2 .
	manualset3
173528	2	413517	7	NULL	NULL	0	NULL	EC	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that EC and CGA have no effect on apoptosis and enhance the intrinsic cellular tolerance against oxidative insults either by activating survival/proliferation pathways or by increasing antioxidant potential in HepG2 .
	manualset3
173529	3	413517	7	NULL	NULL	0	NULL	CGA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that EC and CGA have no effect on apoptosis and enhance the intrinsic cellular tolerance against oxidative insults either by activating survival/proliferation pathways or by increasing antioxidant potential in HepG2 .
	manualset3
173530	4	413517	7	NULL	NULL	0	NULL	effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that EC and CGA have no effect on apoptosis and enhance the intrinsic cellular tolerance against oxidative insults either by activating survival/proliferation pathways or by increasing antioxidant potential in HepG2 .
	manualset3
173531	5	413517	7	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that EC and CGA have no effect on apoptosis and enhance the intrinsic cellular tolerance against oxidative insults either by activating survival/proliferation pathways or by increasing antioxidant potential in HepG2 .
	manualset3
173532	6	413517	7	NULL	NULL	0	NULL	intrinsic cellular tolerance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that EC and CGA have no effect on apoptosis and enhance the intrinsic cellular tolerance against oxidative insults either by activating survival/proliferation pathways or by increasing antioxidant potential in HepG2 .
	manualset3
173533	7	413517	7	NULL	NULL	0	NULL	oxidative insults	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that EC and CGA have no effect on apoptosis and enhance the intrinsic cellular tolerance against oxidative insults either by activating survival/proliferation pathways or by increasing antioxidant potential in HepG2 .
	manualset3
173534	8	413517	7	NULL	NULL	0	NULL	survival/proliferation pathways	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that EC and CGA have no effect on apoptosis and enhance the intrinsic cellular tolerance against oxidative insults either by activating survival/proliferation pathways or by increasing antioxidant potential in HepG2 .
	manualset3
173535	9	413517	7	NULL	NULL	0	NULL	antioxidant potential	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that EC and CGA have no effect on apoptosis and enhance the intrinsic cellular tolerance against oxidative insults either by activating survival/proliferation pathways or by increasing antioxidant potential in HepG2 .
	manualset3
173536	10	413517	7	NULL	NULL	NULL	NULL	HepG2	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data suggest that EC and CGA have no effect on apoptosis and enhance the intrinsic cellular tolerance against oxidative insults either by activating survival/proliferation pathways or by increasing antioxidant potential in HepG2 .
	manualset3
173537	1	413518	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that HSF4 acts as a critical transcription factor for lens-specific target gene expression , in particular regulating the small 25 kDa heat shock protein that acts as a modifier for lens opacity and cataract development .
	manualset3
173538	2	413518	7	NULL	NULL	0	NULL	HSF4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that HSF4 acts as a critical transcription factor for lens-specific target gene expression , in particular regulating the small 25 kDa heat shock protein that acts as a modifier for lens opacity and cataract development .
	manualset3
173539	3	413518	7	NULL	NULL	0	NULL	transcription factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that HSF4 acts as a critical transcription factor for lens-specific target gene expression , in particular regulating the small 25 kDa heat shock protein that acts as a modifier for lens opacity and cataract development .
	manualset3
173540	4	413518	7	NULL	NULL	0	NULL	lens-specific target gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that HSF4 acts as a critical transcription factor for lens-specific target gene expression , in particular regulating the small 25 kDa heat shock protein that acts as a modifier for lens opacity and cataract development .
	manualset3
173541	5	413518	7	NULL	NULL	0	NULL	25 kDa heat shock protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that HSF4 acts as a critical transcription factor for lens-specific target gene expression , in particular regulating the small 25 kDa heat shock protein that acts as a modifier for lens opacity and cataract development .
	manualset3
173542	6	413518	7	NULL	NULL	0	NULL	lens opacity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that HSF4 acts as a critical transcription factor for lens-specific target gene expression , in particular regulating the small 25 kDa heat shock protein that acts as a modifier for lens opacity and cataract development .
	manualset3
173543	7	413518	7	NULL	NULL	0	NULL	cataract development	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that HSF4 acts as a critical transcription factor for lens-specific target gene expression , in particular regulating the small 25 kDa heat shock protein that acts as a modifier for lens opacity and cataract development .
	manualset3
173544	8	413518	7	NULL	NULL	0	NULL	modifier	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that HSF4 acts as a critical transcription factor for lens-specific target gene expression , in particular regulating the small 25 kDa heat shock protein that acts as a modifier for lens opacity and cataract development .
	manualset3
173545	1	413519	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that Kupffer cells but not neutrophils induce an adaptive hepatocellular stress response after hemorrhage and resuscitation .
	manualset3
173546	2	413519	7	NULL	NULL	0	NULL	Kupffer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that Kupffer cells but not neutrophils induce an adaptive hepatocellular stress response after hemorrhage and resuscitation .
	manualset3
173547	3	413519	7	NULL	NULL	NULL	NULL	neutrophils	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data suggest that Kupffer cells but not neutrophils induce an adaptive hepatocellular stress response after hemorrhage and resuscitation .
	manualset3
173548	4	413519	7	NULL	NULL	0	NULL	adaptive hepatocellular stress response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that Kupffer cells but not neutrophils induce an adaptive hepatocellular stress response after hemorrhage and resuscitation .
	manualset3
173549	5	413519	7	NULL	NULL	0	NULL	hemorrhage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that Kupffer cells but not neutrophils induce an adaptive hepatocellular stress response after hemorrhage and resuscitation .
	manualset3
173550	6	413519	7	NULL	NULL	0	NULL	resuscitation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that Kupffer cells but not neutrophils induce an adaptive hepatocellular stress response after hemorrhage and resuscitation .
	manualset3
173551	1	413520	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that Mfn-1 deletion confers protection against ROS-induced mitochondrial dysfunction .
	manualset3
173552	2	413520	7	NULL	NULL	0	NULL	Mfn-1 deletion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that Mfn-1 deletion confers protection against ROS-induced mitochondrial dysfunction .
	manualset3
173553	3	413520	7	NULL	NULL	0	NULL	ROS-induced mitochondrial dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that Mfn-1 deletion confers protection against ROS-induced mitochondrial dysfunction .
	manualset3
173554	1	413521	7	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that Phaenicia sericata can learn a visual pattern with one eye region and later recognize the same pattern with another eye region .
	manualset3
173555	2	413521	7	NULL	NULL	0	NULL	Phaenicia sericata	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that Phaenicia sericata can learn a visual pattern with one eye region and later recognize the same pattern with another eye region .
	manualset3
173556	3	413521	7	NULL	NULL	0	NULL	visual pattern	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that Phaenicia sericata can learn a visual pattern with one eye region and later recognize the same pattern with another eye region .
	manualset3
173557	4	413521	7	NULL	NULL	0	NULL	one eye region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that Phaenicia sericata can learn a visual pattern with one eye region and later recognize the same pattern with another eye region .
	manualset3
173558	5	413521	7	NULL	NULL	0	NULL	pattern	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that Phaenicia sericata can learn a visual pattern with one eye region and later recognize the same pattern with another eye region .
	manualset3
173559	6	413521	7	NULL	NULL	0	NULL	 eye region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that Phaenicia sericata can learn a visual pattern with one eye region and later recognize the same pattern with another eye region .
	manualset3
173560	1	413522	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that SC in human milk binds to toxin A and may function as a receptor analog , protecting human infants against C. difficile-associated disease .
	manualset3
173561	2	413522	7	NULL	NULL	0	NULL	SC	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that SC in human milk binds to toxin A and may function as a receptor analog , protecting human infants against C. difficile-associated disease .
	manualset3
173562	3	413522	7	NULL	NULL	0	NULL	human milk 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that SC in human milk binds to toxin A and may function as a receptor analog , protecting human infants against C. difficile-associated disease .
	manualset3
173563	4	413522	7	NULL	NULL	0	NULL	toxin A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that SC in human milk binds to toxin A and may function as a receptor analog , protecting human infants against C. difficile-associated disease .
	manualset3
173564	5	413522	7	NULL	NULL	0	NULL	 receptor analog	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that SC in human milk binds to toxin A and may function as a receptor analog , protecting human infants against C. difficile-associated disease .
	manualset3
173565	6	413522	7	NULL	NULL	0	NULL	human infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that SC in human milk binds to toxin A and may function as a receptor analog , protecting human infants against C. difficile-associated disease .
	manualset3
173566	7	413522	7	NULL	NULL	0	NULL	C. difficile-associated disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that SC in human milk binds to toxin A and may function as a receptor analog , protecting human infants against C. difficile-associated disease .
	manualset3
173567	1	413523	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that Tregs contribute to viral persistence .
	manualset3
173568	2	413523	7	NULL	NULL	0	NULL	Tregs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that Tregs contribute to viral persistence .
	manualset3
173569	3	413523	7	NULL	NULL	0	NULL	viral persistence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that Tregs contribute to viral persistence .
	manualset3
173570	1	413524	7	NULL	NULL	0	NULL	Acute retinal necrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute retinal necrosis features , management , and outcomes .
	manualset3
173571	2	413524	7	NULL	NULL	0	NULL	management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute retinal necrosis features , management , and outcomes .
	manualset3
173572	3	413524	7	NULL	NULL	0	NULL	outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute retinal necrosis features , management , and outcomes .
	manualset3
173573	1	413525	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that UCH L1 , with avidity and affinity for ubiquitin , insures ubiquitin stability within neurons .
	manualset3
173574	2	413525	7	NULL	NULL	0	NULL	UCH L1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that UCH L1 , with avidity and affinity for ubiquitin , insures ubiquitin stability within neurons .
	manualset3
173575	3	413525	7	NULL	NULL	0	NULL	avidity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that UCH L1 , with avidity and affinity for ubiquitin , insures ubiquitin stability within neurons .
	manualset3
173576	4	413525	7	NULL	NULL	0	NULL	affinity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that UCH L1 , with avidity and affinity for ubiquitin , insures ubiquitin stability within neurons .
	manualset3
173577	5	413525	7	NULL	NULL	0	NULL	ubiquitin	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that UCH L1 , with avidity and affinity for ubiquitin , insures ubiquitin stability within neurons .
	manualset3
173578	6	413525	7	NULL	NULL	0	NULL	ubiquitin stability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that UCH L1 , with avidity and affinity for ubiquitin , insures ubiquitin stability within neurons .
	manualset3
173579	7	413525	7	NULL	NULL	0	NULL	neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that UCH L1 , with avidity and affinity for ubiquitin , insures ubiquitin stability within neurons .
	manualset3
173580	1	413526	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that during virus infection , the compartments in the secretory pathway , such as the endoplasmic reticulum ( ER ) and Golgi complex , are major sites of accumulation of the SH protein .
	manualset3
173581	2	413526	7	NULL	NULL	0	NULL	virus infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that during virus infection , the compartments in the secretory pathway , such as the endoplasmic reticulum ( ER ) and Golgi complex , are major sites of accumulation of the SH protein .
	manualset3
173582	3	413526	7	NULL	NULL	0	NULL	compartments	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that during virus infection , the compartments in the secretory pathway , such as the endoplasmic reticulum ( ER ) and Golgi complex , are major sites of accumulation of the SH protein .
	manualset3
173583	4	413526	7	NULL	NULL	0	NULL	secretory pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that during virus infection , the compartments in the secretory pathway , such as the endoplasmic reticulum ( ER ) and Golgi complex , are major sites of accumulation of the SH protein .
	manualset3
173584	5	413526	7	NULL	NULL	0	NULL	endoplasmic reticulum ( ER )	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that during virus infection , the compartments in the secretory pathway , such as the endoplasmic reticulum ( ER ) and Golgi complex , are major sites of accumulation of the SH protein .
	manualset3
173585	6	413526	7	NULL	NULL	0	NULL	Golgi complex	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that during virus infection , the compartments in the secretory pathway , such as the endoplasmic reticulum ( ER ) and Golgi complex , are major sites of accumulation of the SH protein .
	manualset3
173586	7	413526	7	NULL	NULL	0	NULL	major sites	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that during virus infection , the compartments in the secretory pathway , such as the endoplasmic reticulum ( ER ) and Golgi complex , are major sites of accumulation of the SH protein .
	manualset3
173587	8	413526	7	NULL	NULL	0	NULL	accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that during virus infection , the compartments in the secretory pathway , such as the endoplasmic reticulum ( ER ) and Golgi complex , are major sites of accumulation of the SH protein .
	manualset3
173588	9	413526	7	NULL	NULL	0	NULL	SH protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that during virus infection , the compartments in the secretory pathway , such as the endoplasmic reticulum ( ER ) and Golgi complex , are major sites of accumulation of the SH protein .
	manualset3
173589	1	413527	7	NULL	NULL	0	NULL	 data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that in addition to its well-documented antiproliferative effects , IFN-alpha can inhibit the growth of human bladder cancer cells by inhibition of angiogenesis .
	manualset3
173590	2	413527	7	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that in addition to its well-documented antiproliferative effects , IFN-alpha can inhibit the growth of human bladder cancer cells by inhibition of angiogenesis .
	manualset3
173591	3	413527	7	NULL	NULL	0	NULL	antiproliferative effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that in addition to its well-documented antiproliferative effects , IFN-alpha can inhibit the growth of human bladder cancer cells by inhibition of angiogenesis .
	manualset3
173592	4	413527	7	NULL	NULL	0	NULL	IFN-alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that in addition to its well-documented antiproliferative effects , IFN-alpha can inhibit the growth of human bladder cancer cells by inhibition of angiogenesis .
	manualset3
173593	5	413527	7	NULL	NULL	0	NULL	 growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that in addition to its well-documented antiproliferative effects , IFN-alpha can inhibit the growth of human bladder cancer cells by inhibition of angiogenesis .
	manualset3
173594	6	413527	7	NULL	NULL	0	NULL	human bladder cancer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that in addition to its well-documented antiproliferative effects , IFN-alpha can inhibit the growth of human bladder cancer cells by inhibition of angiogenesis .
	manualset3
173595	7	413527	7	NULL	NULL	0	NULL	 inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that in addition to its well-documented antiproliferative effects , IFN-alpha can inhibit the growth of human bladder cancer cells by inhibition of angiogenesis .
	manualset3
173596	8	413527	7	NULL	NULL	0	NULL	angiogenesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that in addition to its well-documented antiproliferative effects , IFN-alpha can inhibit the growth of human bladder cancer cells by inhibition of angiogenesis .
	manualset3
173597	1	413528	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that increases in TNF-alpha may cause insulin resistance in skeletal muscle by inhibiting IRS-1 - and IRS-2-mediated PI 3-kinase activation as well as p42 ( MAPK ) and p44 ( MAPK ) tyrosine phosphorylation , leading to impaired insulin-stimulated glucose uptake .
	manualset3
173598	2	413528	7	NULL	NULL	0	NULL	TNF-alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that increases in TNF-alpha may cause insulin resistance in skeletal muscle by inhibiting IRS-1 - and IRS-2-mediated PI 3-kinase activation as well as p42 ( MAPK ) and p44 ( MAPK ) tyrosine phosphorylation , leading to impaired insulin-stimulated glucose uptake .
	manualset3
173599	3	413528	7	NULL	NULL	NULL	NULL	 insulin resistance	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data suggest that increases in TNF-alpha may cause insulin resistance in skeletal muscle by inhibiting IRS-1 - and IRS-2-mediated PI 3-kinase activation as well as p42 ( MAPK ) and p44 ( MAPK ) tyrosine phosphorylation , leading to impaired insulin-stimulated glucose uptake .
	manualset3
173600	4	413528	7	NULL	NULL	0	NULL	skeletal muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that increases in TNF-alpha may cause insulin resistance in skeletal muscle by inhibiting IRS-1 - and IRS-2-mediated PI 3-kinase activation as well as p42 ( MAPK ) and p44 ( MAPK ) tyrosine phosphorylation , leading to impaired insulin-stimulated glucose uptake .
	manualset3
173601	5	413528	7	NULL	NULL	0	NULL	IRS-1 -mediated PI 3-kinase activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that increases in TNF-alpha may cause insulin resistance in skeletal muscle by inhibiting IRS-1 - and IRS-2-mediated PI 3-kinase activation as well as p42 ( MAPK ) and p44 ( MAPK ) tyrosine phosphorylation , leading to impaired insulin-stimulated glucose uptake .
	manualset3
173602	6	413528	7	NULL	NULL	0	NULL	IRS-2-mediated PI 3-kinase activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that increases in TNF-alpha may cause insulin resistance in skeletal muscle by inhibiting IRS-1 - and IRS-2-mediated PI 3-kinase activation as well as p42 ( MAPK ) and p44 ( MAPK ) tyrosine phosphorylation , leading to impaired insulin-stimulated glucose uptake .
	manualset3
173603	7	413528	7	NULL	NULL	0	NULL	p42 ( MAPK )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that increases in TNF-alpha may cause insulin resistance in skeletal muscle by inhibiting IRS-1 - and IRS-2-mediated PI 3-kinase activation as well as p42 ( MAPK ) and p44 ( MAPK ) tyrosine phosphorylation , leading to impaired insulin-stimulated glucose uptake .
	manualset3
173604	8	413528	7	NULL	NULL	0	NULL	p44 ( MAPK ) tyrosine phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that increases in TNF-alpha may cause insulin resistance in skeletal muscle by inhibiting IRS-1 - and IRS-2-mediated PI 3-kinase activation as well as p42 ( MAPK ) and p44 ( MAPK ) tyrosine phosphorylation , leading to impaired insulin-stimulated glucose uptake .
	manualset3
173605	9	413528	7	NULL	NULL	0	NULL	insulin-stimulated glucose uptake	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that increases in TNF-alpha may cause insulin resistance in skeletal muscle by inhibiting IRS-1 - and IRS-2-mediated PI 3-kinase activation as well as p42 ( MAPK ) and p44 ( MAPK ) tyrosine phosphorylation , leading to impaired insulin-stimulated glucose uptake .
	manualset3
173606	1	413529	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that inhibition of PI-PLC may account , in part , for the anti-inflammatory actions of manoalide .
	manualset3
173607	2	413529	7	NULL	NULL	0	NULL	inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that inhibition of PI-PLC may account , in part , for the anti-inflammatory actions of manoalide .
	manualset3
173608	3	413529	7	NULL	NULL	0	NULL	PI-PLC 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that inhibition of PI-PLC may account , in part , for the anti-inflammatory actions of manoalide .
	manualset3
173609	4	413529	7	NULL	NULL	0	NULL	anti-inflammatory actions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that inhibition of PI-PLC may account , in part , for the anti-inflammatory actions of manoalide .
	manualset3
173610	5	413529	7	NULL	NULL	0	NULL	manoalide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that inhibition of PI-PLC may account , in part , for the anti-inflammatory actions of manoalide .
	manualset3
173611	1	413530	7	NULL	NULL	0	NULL	 data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that pregnancy is a dynamic state in which CD8 T-cell turnover is increased while the function and ending size of the CD8 T-cell compartment are maintained .
	manualset3
173612	2	413530	7	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that pregnancy is a dynamic state in which CD8 T-cell turnover is increased while the function and ending size of the CD8 T-cell compartment are maintained .
	manualset3
173613	3	413530	7	NULL	NULL	0	NULL	dynamic state	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that pregnancy is a dynamic state in which CD8 T-cell turnover is increased while the function and ending size of the CD8 T-cell compartment are maintained .
	manualset3
173614	4	413530	7	NULL	NULL	0	NULL	CD8 T-cell turnover	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that pregnancy is a dynamic state in which CD8 T-cell turnover is increased while the function and ending size of the CD8 T-cell compartment are maintained .
	manualset3
173615	5	413530	7	NULL	NULL	0	NULL	function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that pregnancy is a dynamic state in which CD8 T-cell turnover is increased while the function and ending size of the CD8 T-cell compartment are maintained .
	manualset3
173616	6	413530	7	NULL	NULL	0	NULL	ending size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that pregnancy is a dynamic state in which CD8 T-cell turnover is increased while the function and ending size of the CD8 T-cell compartment are maintained .
	manualset3
173617	7	413530	7	NULL	NULL	0	NULL	CD8 T-cell compartment	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that pregnancy is a dynamic state in which CD8 T-cell turnover is increased while the function and ending size of the CD8 T-cell compartment are maintained .
	manualset3
173657	1	413531	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that small platform stress induces hypersensitivity of mice to the motor depressant effect of baclofen .
	manualset3
173658	2	413531	7	NULL	NULL	NULL	NULL	small platform stress	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data suggest that small platform stress induces hypersensitivity of mice to the motor depressant effect of baclofen .
	manualset3
173659	3	413531	7	NULL	NULL	NULL	NULL	hypersensitivity 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data suggest that small platform stress induces hypersensitivity of mice to the motor depressant effect of baclofen .
	manualset3
173660	4	413531	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that small platform stress induces hypersensitivity of mice to the motor depressant effect of baclofen .
	manualset3
173661	5	413531	7	NULL	NULL	0	NULL	motor depressant effect 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that small platform stress induces hypersensitivity of mice to the motor depressant effect of baclofen .
	manualset3
173662	6	413531	7	NULL	NULL	0	NULL	baclofen	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that small platform stress induces hypersensitivity of mice to the motor depressant effect of baclofen .
	manualset3
173663	1	413532	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that the addition of alpha1-AT to surfactant can exert a positive effect on oxygenation and surfactant metabolism in surfactant-deficient rats .
	manualset3
173664	2	413532	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that the addition of alpha1-AT to surfactant can exert a positive effect on oxygenation and surfactant metabolism in surfactant-deficient rats .
	manualset3
173665	3	413532	7	NULL	NULL	0	NULL	alpha1-AT	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that the addition of alpha1-AT to surfactant can exert a positive effect on oxygenation and surfactant metabolism in surfactant-deficient rats .
	manualset3
173666	4	413532	7	NULL	NULL	0	NULL	surfactant	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that the addition of alpha1-AT to surfactant can exert a positive effect on oxygenation and surfactant metabolism in surfactant-deficient rats .
	manualset3
173667	5	413532	7	NULL	NULL	0	NULL	positive effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that the addition of alpha1-AT to surfactant can exert a positive effect on oxygenation and surfactant metabolism in surfactant-deficient rats .
	manualset3
173668	6	413532	7	NULL	NULL	0	NULL	oxygenation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that the addition of alpha1-AT to surfactant can exert a positive effect on oxygenation and surfactant metabolism in surfactant-deficient rats .
	manualset3
173669	7	413532	7	NULL	NULL	0	NULL	surfactant metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that the addition of alpha1-AT to surfactant can exert a positive effect on oxygenation and surfactant metabolism in surfactant-deficient rats .
	manualset3
173670	8	413532	7	NULL	NULL	0	NULL	surfactant-deficient rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that the addition of alpha1-AT to surfactant can exert a positive effect on oxygenation and surfactant metabolism in surfactant-deficient rats .
	manualset3
173671	1	413533	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that the whale relied on cues relevant to target shape as well as target strength , that changes in source level and bandwidth were task-related , that the decrease in clicks was associated with learning experience , and that Pseudorca 's ability to discriminate shapes using echolocation may be comparable to that of Tursiops truncatus .
	manualset3
173672	2	413533	7	NULL	NULL	0	NULL	 whale	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that the whale relied on cues relevant to target shape as well as target strength , that changes in source level and bandwidth were task-related , that the decrease in clicks was associated with learning experience , and that Pseudorca 's ability to discriminate shapes using echolocation may be comparable to that of Tursiops truncatus .
	manualset3
173673	3	413533	7	NULL	NULL	0	NULL	cues	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that the whale relied on cues relevant to target shape as well as target strength , that changes in source level and bandwidth were task-related , that the decrease in clicks was associated with learning experience , and that Pseudorca 's ability to discriminate shapes using echolocation may be comparable to that of Tursiops truncatus .
	manualset3
173680	4	413533	7	NULL	NULL	0	NULL	target shape	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that the whale relied on cues relevant to target shape as well as target strength , that changes in source level and bandwidth were task-related , that the decrease in clicks was associated with learning experience , and that Pseudorca 's ability to discriminate shapes using echolocation may be comparable to that of Tursiops truncatus .
	manualset3
173682	5	413533	7	NULL	NULL	0	NULL	 target strength	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that the whale relied on cues relevant to target shape as well as target strength , that changes in source level and bandwidth were task-related , that the decrease in clicks was associated with learning experience , and that Pseudorca 's ability to discriminate shapes using echolocation may be comparable to that of Tursiops truncatus .
	manualset3
173690	7	413533	7	NULL	NULL	NULL	NULL	source level	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data suggest that the whale relied on cues relevant to target shape as well as target strength , that changes in source level and bandwidth were task-related , that the decrease in clicks was associated with learning experience , and that Pseudorca 's ability to discriminate shapes using echolocation may be comparable to that of Tursiops truncatus .
	manualset3
173695	8	413533	7	NULL	NULL	NULL	NULL	bandwidth	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data suggest that the whale relied on cues relevant to target shape as well as target strength , that changes in source level and bandwidth were task-related , that the decrease in clicks was associated with learning experience , and that Pseudorca 's ability to discriminate shapes using echolocation may be comparable to that of Tursiops truncatus .
	manualset3
173696	9	413533	7	NULL	NULL	0	NULL	decrease	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that the whale relied on cues relevant to target shape as well as target strength , that changes in source level and bandwidth were task-related , that the decrease in clicks was associated with learning experience , and that Pseudorca 's ability to discriminate shapes using echolocation may be comparable to that of Tursiops truncatus .
	manualset3
173697	10	413533	7	NULL	NULL	0	NULL	clicks	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that the whale relied on cues relevant to target shape as well as target strength , that changes in source level and bandwidth were task-related , that the decrease in clicks was associated with learning experience , and that Pseudorca 's ability to discriminate shapes using echolocation may be comparable to that of Tursiops truncatus .
	manualset3
173698	11	413533	7	NULL	NULL	0	NULL	learning experience	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that the whale relied on cues relevant to target shape as well as target strength , that changes in source level and bandwidth were task-related , that the decrease in clicks was associated with learning experience , and that Pseudorca 's ability to discriminate shapes using echolocation may be comparable to that of Tursiops truncatus .
	manualset3
173699	12	413533	7	NULL	NULL	0	NULL	Pseudorca 's ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that the whale relied on cues relevant to target shape as well as target strength , that changes in source level and bandwidth were task-related , that the decrease in clicks was associated with learning experience , and that Pseudorca 's ability to discriminate shapes using echolocation may be comparable to that of Tursiops truncatus .
	manualset3
173700	13	413533	7	NULL	NULL	0	NULL	shapes	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that the whale relied on cues relevant to target shape as well as target strength , that changes in source level and bandwidth were task-related , that the decrease in clicks was associated with learning experience , and that Pseudorca 's ability to discriminate shapes using echolocation may be comparable to that of Tursiops truncatus .
	manualset3
173701	14	413533	7	NULL	NULL	NULL	NULL	echolocation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data suggest that the whale relied on cues relevant to target shape as well as target strength , that changes in source level and bandwidth were task-related , that the decrease in clicks was associated with learning experience , and that Pseudorca 's ability to discriminate shapes using echolocation may be comparable to that of Tursiops truncatus .
	manualset3
173702	15	413533	7	NULL	NULL	0	NULL	Tursiops truncatus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggest that the whale relied on cues relevant to target shape as well as target strength , that changes in source level and bandwidth were task-related , that the decrease in clicks was associated with learning experience , and that Pseudorca 's ability to discriminate shapes using echolocation may be comparable to that of Tursiops truncatus .
	manualset3
173703	1	413534	7	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggested that RGD peptide may have the potential to prevent PCO .
	manualset3
173704	2	413534	7	NULL	NULL	0	NULL	RGD peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggested that RGD peptide may have the potential to prevent PCO .
	manualset3
173705	3	413534	7	NULL	NULL	0	NULL	potential	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggested that RGD peptide may have the potential to prevent PCO .
	manualset3
173706	4	413534	7	NULL	NULL	0	NULL	PCO	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggested that RGD peptide may have the potential to prevent PCO .
	manualset3
173707	1	413535	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggested that behavioral alleviation with EA stimulation may be associated with modulation of neurotransmitters release , such as Glu and ACh in the striatum , rather than with DA restoration .
	manualset3
173708	2	413535	7	NULL	NULL	0	NULL	behavioral alleviation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggested that behavioral alleviation with EA stimulation may be associated with modulation of neurotransmitters release , such as Glu and ACh in the striatum , rather than with DA restoration .
	manualset3
173709	3	413535	7	NULL	NULL	NULL	NULL	EA stimulation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data suggested that behavioral alleviation with EA stimulation may be associated with modulation of neurotransmitters release , such as Glu and ACh in the striatum , rather than with DA restoration .
	manualset3
173710	4	413535	7	NULL	NULL	NULL	NULL	modulation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data suggested that behavioral alleviation with EA stimulation may be associated with modulation of neurotransmitters release , such as Glu and ACh in the striatum , rather than with DA restoration .
	manualset3
173711	5	413535	7	NULL	NULL	0	NULL	neurotransmitters release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggested that behavioral alleviation with EA stimulation may be associated with modulation of neurotransmitters release , such as Glu and ACh in the striatum , rather than with DA restoration .
	manualset3
173712	6	413535	7	NULL	NULL	0	NULL	Glu	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggested that behavioral alleviation with EA stimulation may be associated with modulation of neurotransmitters release , such as Glu and ACh in the striatum , rather than with DA restoration .
	manualset3
173713	7	413535	7	NULL	NULL	0	NULL	ACh	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggested that behavioral alleviation with EA stimulation may be associated with modulation of neurotransmitters release , such as Glu and ACh in the striatum , rather than with DA restoration .
	manualset3
173714	8	413535	7	NULL	NULL	0	NULL	 striatum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggested that behavioral alleviation with EA stimulation may be associated with modulation of neurotransmitters release , such as Glu and ACh in the striatum , rather than with DA restoration .
	manualset3
173715	9	413535	7	NULL	NULL	0	NULL	DA restoration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data suggested that behavioral alleviation with EA stimulation may be associated with modulation of neurotransmitters release , such as Glu and ACh in the striatum , rather than with DA restoration .
	manualset3
173716	1	413536	7	NULL	NULL	0	NULL	 data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support a role for the circadian clock protein Per1 in the coordinate regulation of genes involved in renal sodium reabsorption .
	manualset3
173717	2	413536	7	NULL	NULL	0	NULL	 role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support a role for the circadian clock protein Per1 in the coordinate regulation of genes involved in renal sodium reabsorption .
	manualset3
173718	3	413536	7	NULL	NULL	0	NULL	circadian clock protein Per1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support a role for the circadian clock protein Per1 in the coordinate regulation of genes involved in renal sodium reabsorption .
	manualset3
173719	4	413536	7	NULL	NULL	0	NULL	coordinate regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support a role for the circadian clock protein Per1 in the coordinate regulation of genes involved in renal sodium reabsorption .
	manualset3
173720	5	413536	7	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support a role for the circadian clock protein Per1 in the coordinate regulation of genes involved in renal sodium reabsorption .
	manualset3
173721	6	413536	7	NULL	NULL	0	NULL	renal sodium reabsorption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support a role for the circadian clock protein Per1 in the coordinate regulation of genes involved in renal sodium reabsorption .
	manualset3
173722	1	413537	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support the concept that tissue injury that is complement and neutrophil dependent may be related to generation of OH .
	manualset3
173723	2	413537	7	NULL	NULL	0	NULL	concept	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support the concept that tissue injury that is complement and neutrophil dependent may be related to generation of OH .
	manualset3
173724	3	413537	7	NULL	NULL	0	NULL	tissue injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support the concept that tissue injury that is complement and neutrophil dependent may be related to generation of OH .
	manualset3
173725	4	413537	7	NULL	NULL	NULL	NULL	complement dependent	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data support the concept that tissue injury that is complement and neutrophil dependent may be related to generation of OH .
	manualset3
173726	5	413537	7	NULL	NULL	NULL	NULL	neutrophil dependent	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data support the concept that tissue injury that is complement and neutrophil dependent may be related to generation of OH .
	manualset3
173727	6	413537	7	NULL	NULL	0	NULL	generation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support the concept that tissue injury that is complement and neutrophil dependent may be related to generation of OH .
	manualset3
173728	7	413537	7	NULL	NULL	0	NULL	OH	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support the concept that tissue injury that is complement and neutrophil dependent may be related to generation of OH .
	manualset3
173729	1	413538	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support the conclusion that L-selectin , but not E-selectin , can signal the transition from neutrophil rolling to cell arrest under shear flow .
	manualset3
173730	2	413538	7	NULL	NULL	0	NULL	conclusion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support the conclusion that L-selectin , but not E-selectin , can signal the transition from neutrophil rolling to cell arrest under shear flow .
	manualset3
173731	3	413538	7	NULL	NULL	0	NULL	L-selectin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support the conclusion that L-selectin , but not E-selectin , can signal the transition from neutrophil rolling to cell arrest under shear flow .
	manualset3
173732	4	413538	7	NULL	NULL	0	NULL	E-selectin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support the conclusion that L-selectin , but not E-selectin , can signal the transition from neutrophil rolling to cell arrest under shear flow .
	manualset3
173733	5	413538	7	NULL	NULL	NULL	NULL	transition	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data support the conclusion that L-selectin , but not E-selectin , can signal the transition from neutrophil rolling to cell arrest under shear flow .
	manualset3
173734	6	413538	7	NULL	NULL	0	NULL	neutrophil	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support the conclusion that L-selectin , but not E-selectin , can signal the transition from neutrophil rolling to cell arrest under shear flow .
	manualset3
173735	7	413538	7	NULL	NULL	0	NULL	cell arrest	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support the conclusion that L-selectin , but not E-selectin , can signal the transition from neutrophil rolling to cell arrest under shear flow .
	manualset3
173736	8	413538	7	NULL	NULL	0	NULL	shear flow 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support the conclusion that L-selectin , but not E-selectin , can signal the transition from neutrophil rolling to cell arrest under shear flow .
	manualset3
173737	1	413539	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support the hypothesis that in the epileptic human hippocampus , there may be pathophysiologic associations among mossy fiber synaptic plasticity , hippocampal neuron damage , and granule cell mRNA neurotrophin levels .
	manualset3
173738	2	413539	7	NULL	NULL	NULL	NULL	hypothesis	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data support the hypothesis that in the epileptic human hippocampus , there may be pathophysiologic associations among mossy fiber synaptic plasticity , hippocampal neuron damage , and granule cell mRNA neurotrophin levels .
	manualset3
173739	3	413539	7	NULL	NULL	0	NULL	epileptic human hippocampus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support the hypothesis that in the epileptic human hippocampus , there may be pathophysiologic associations among mossy fiber synaptic plasticity , hippocampal neuron damage , and granule cell mRNA neurotrophin levels .
	manualset3
173740	4	413539	7	NULL	NULL	0	NULL	pathophysiologic associations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support the hypothesis that in the epileptic human hippocampus , there may be pathophysiologic associations among mossy fiber synaptic plasticity , hippocampal neuron damage , and granule cell mRNA neurotrophin levels .
	manualset3
173741	5	413539	7	NULL	NULL	0	NULL	mossy fiber synaptic plasticity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support the hypothesis that in the epileptic human hippocampus , there may be pathophysiologic associations among mossy fiber synaptic plasticity , hippocampal neuron damage , and granule cell mRNA neurotrophin levels .
	manualset3
173742	6	413539	7	NULL	NULL	0	NULL	hippocampal neuron damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support the hypothesis that in the epileptic human hippocampus , there may be pathophysiologic associations among mossy fiber synaptic plasticity , hippocampal neuron damage , and granule cell mRNA neurotrophin levels .
	manualset3
173743	7	413539	7	NULL	NULL	NULL	NULL	granule cell mRNA neurotrophin levels	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data support the hypothesis that in the epileptic human hippocampus , there may be pathophysiologic associations among mossy fiber synaptic plasticity , hippocampal neuron damage , and granule cell mRNA neurotrophin levels .
	manualset3
173744	1	413540	7	NULL	NULL	0	NULL	 data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support the possibility that increased dopamine transmission in the VTA is involved in the cellular events that determine the initiation of behavioral sensitization to cocaine .
	manualset3
173746	3	413540	7	NULL	NULL	0	NULL	possibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support the possibility that increased dopamine transmission in the VTA is involved in the cellular events that determine the initiation of behavioral sensitization to cocaine .
	manualset3
173747	4	413540	7	NULL	NULL	0	NULL	dopamine transmission	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support the possibility that increased dopamine transmission in the VTA is involved in the cellular events that determine the initiation of behavioral sensitization to cocaine .
	manualset3
173748	5	413540	7	NULL	NULL	0	NULL	VTA	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support the possibility that increased dopamine transmission in the VTA is involved in the cellular events that determine the initiation of behavioral sensitization to cocaine .
	manualset3
173749	6	413540	7	NULL	NULL	0	NULL	cellular events	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support the possibility that increased dopamine transmission in the VTA is involved in the cellular events that determine the initiation of behavioral sensitization to cocaine .
	manualset3
173750	7	413540	7	NULL	NULL	0	NULL	initiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support the possibility that increased dopamine transmission in the VTA is involved in the cellular events that determine the initiation of behavioral sensitization to cocaine .
	manualset3
173751	8	413540	7	NULL	NULL	0	NULL	behavioral sensitization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support the possibility that increased dopamine transmission in the VTA is involved in the cellular events that determine the initiation of behavioral sensitization to cocaine .
	manualset3
173752	9	413540	7	NULL	NULL	0	NULL	cocaine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support the possibility that increased dopamine transmission in the VTA is involved in the cellular events that determine the initiation of behavioral sensitization to cocaine .
	manualset3
173753	1	413541	7	NULL	NULL	0	NULL	Acute thrombosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute thrombosis of an abdominal aneurysm is a catastrophic complication which is little known .
	manualset3
173754	2	413541	7	NULL	NULL	0	NULL	abdominal aneurysm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute thrombosis of an abdominal aneurysm is a catastrophic complication which is little known .
	manualset3
173755	3	413541	7	NULL	NULL	0	NULL	catastrophic complication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute thrombosis of an abdominal aneurysm is a catastrophic complication which is little known .
	manualset3
173756	1	413542	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data taken together , led us to conclude that differential alteration in ET expression and its receptors may be mediated by TNF - and may , in part , account for the pathogenesis of acute lung injury in endotoxemia .
	manualset3
173757	2	413542	7	NULL	NULL	0	NULL	differential alteration	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data taken together , led us to conclude that differential alteration in ET expression and its receptors may be mediated by TNF - and may , in part , account for the pathogenesis of acute lung injury in endotoxemia .
	manualset3
173758	3	413542	7	NULL	NULL	0	NULL	ET expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data taken together , led us to conclude that differential alteration in ET expression and its receptors may be mediated by TNF - and may , in part , account for the pathogenesis of acute lung injury in endotoxemia .
	manualset3
173759	4	413542	7	NULL	NULL	0	NULL	receptors 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data taken together , led us to conclude that differential alteration in ET expression and its receptors may be mediated by TNF - and may , in part , account for the pathogenesis of acute lung injury in endotoxemia .
	manualset3
173760	5	413542	7	NULL	NULL	NULL	NULL	TNF	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These data taken together , led us to conclude that differential alteration in ET expression and its receptors may be mediated by TNF - and may , in part , account for the pathogenesis of acute lung injury in endotoxemia .
	manualset3
173761	6	413542	7	NULL	NULL	0	NULL	pathogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data taken together , led us to conclude that differential alteration in ET expression and its receptors may be mediated by TNF - and may , in part , account for the pathogenesis of acute lung injury in endotoxemia .
	manualset3
173762	7	413542	7	NULL	NULL	0	NULL	acute lung injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These data taken together , led us to conclude that differential alteration in ET expression and its receptors may be mediated by TNF - and may , in part , account for the pathogenesis of acute lung injury in endotoxemia .
	manualset3
173763	8	413542	7	NULL	NULL	0	NULL	endotoxemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These data taken together , led us to conclude that differential alteration in ET expression and its receptors may be mediated by TNF - and may , in part , account for the pathogenesis of acute lung injury in endotoxemia .
	manualset3
173764	1	413543	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data yield a linear relationship between current and air gap , the slope of which is used to determine average surface-absorbed-dose rate over the central area of the source .
	manualset3
173765	2	413543	7	NULL	NULL	0	NULL	linear relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These data yield a linear relationship between current and air gap , the slope of which is used to determine average surface-absorbed-dose rate over the central area of the source .
	manualset3
173766	3	413543	7	NULL	NULL	0	NULL	current gap	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These data yield a linear relationship between current and air gap , the slope of which is used to determine average surface-absorbed-dose rate over the central area of the source .
	manualset3
173767	4	413543	7	NULL	NULL	0	NULL	air gap	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These data yield a linear relationship between current and air gap , the slope of which is used to determine average surface-absorbed-dose rate over the central area of the source .
	manualset3
173768	5	413543	7	NULL	NULL	0	NULL	slope	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These data yield a linear relationship between current and air gap , the slope of which is used to determine average surface-absorbed-dose rate over the central area of the source .
	manualset3
173769	6	413543	7	NULL	NULL	0	NULL	average surface-absorbed-dose rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data yield a linear relationship between current and air gap , the slope of which is used to determine average surface-absorbed-dose rate over the central area of the source .
	manualset3
173770	7	413543	7	NULL	NULL	0	NULL	central area	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These data yield a linear relationship between current and air gap , the slope of which is used to determine average surface-absorbed-dose rate over the central area of the source .
	manualset3
173771	8	413543	7	NULL	NULL	0	NULL	source	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data yield a linear relationship between current and air gap , the slope of which is used to determine average surface-absorbed-dose rate over the central area of the source .
	manualset3
173772	1	413544	7	NULL	NULL	0	NULL	date	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	These date are confirmed by the finding of higher nutrient concentration and higher energy content of milk formulas , as prepared by mothers .
	manualset3
173773	2	413544	7	NULL	NULL	0	NULL	higher nutrient concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These date are confirmed by the finding of higher nutrient concentration and higher energy content of milk formulas , as prepared by mothers .
	manualset3
173774	3	413544	7	NULL	NULL	0	NULL	higher energy content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These date are confirmed by the finding of higher nutrient concentration and higher energy content of milk formulas , as prepared by mothers .
	manualset3
173775	4	413544	7	NULL	NULL	NULL	NULL	milk formulas 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These date are confirmed by the finding of higher nutrient concentration and higher energy content of milk formulas , as prepared by mothers .
	manualset3
173776	5	413544	7	NULL	NULL	0	NULL	mothers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These date are confirmed by the finding of higher nutrient concentration and higher energy content of milk formulas , as prepared by mothers .
	manualset3
175211	6	413544	7	NULL	NULL	0	NULL	finding	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These date are confirmed by the finding of higher nutrient concentration and higher energy content of milk formulas , as prepared by mothers .
	manualset3
173777	1	413545	7	NULL	NULL	0	NULL	defects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These defects include the formation of additional rosettes originating from axils at the base of the plant as well as aerial rosettes formed at the axils of the first few nodes of the shoot .
	manualset3
173778	2	413545	7	NULL	NULL	0	NULL	formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These defects include the formation of additional rosettes originating from axils at the base of the plant as well as aerial rosettes formed at the axils of the first few nodes of the shoot .
	manualset3
173779	3	413545	7	NULL	NULL	0	NULL	rosettes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These defects include the formation of additional rosettes originating from axils at the base of the plant as well as aerial rosettes formed at the axils of the first few nodes of the shoot .
	manualset3
173780	4	413545	7	NULL	NULL	0	NULL	axils	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These defects include the formation of additional rosettes originating from axils at the base of the plant as well as aerial rosettes formed at the axils of the first few nodes of the shoot .
	manualset3
173781	5	413545	7	NULL	NULL	0	NULL	base of the plant 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These defects include the formation of additional rosettes originating from axils at the base of the plant as well as aerial rosettes formed at the axils of the first few nodes of the shoot .
	manualset3
173782	6	413545	7	NULL	NULL	0	NULL	aerial rosettes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These defects include the formation of additional rosettes originating from axils at the base of the plant as well as aerial rosettes formed at the axils of the first few nodes of the shoot .
	manualset3
173783	7	413545	7	NULL	NULL	0	NULL	axils	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These defects include the formation of additional rosettes originating from axils at the base of the plant as well as aerial rosettes formed at the axils of the first few nodes of the shoot .
	manualset3
173784	8	413545	7	NULL	NULL	0	NULL	first few nodes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These defects include the formation of additional rosettes originating from axils at the base of the plant as well as aerial rosettes formed at the axils of the first few nodes of the shoot .
	manualset3
173785	9	413545	7	NULL	NULL	0	NULL	shoot	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These defects include the formation of additional rosettes originating from axils at the base of the plant as well as aerial rosettes formed at the axils of the first few nodes of the shoot .
	manualset3
173786	1	413546	7	NULL	NULL	NULL	NULL	deposits	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These deposits can be later taken up into the water .
	manualset3
173787	2	413546	7	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These deposits can be later taken up into the water .
	manualset3
173788	1	413547	7	NULL	NULL	0	NULL	deviations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These deviations are addressed by augmenting the model to account for decentralized flow in some microprocessor networks ( e.g. in logic networks ) .
	manualset3
173789	2	413547	7	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These deviations are addressed by augmenting the model to account for decentralized flow in some microprocessor networks ( e.g. in logic networks ) .
	manualset3
173790	3	413547	7	NULL	NULL	0	NULL	decentralized flow	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These deviations are addressed by augmenting the model to account for decentralized flow in some microprocessor networks ( e.g. in logic networks ) .
	manualset3
173791	4	413547	7	NULL	NULL	0	NULL	microprocessor networks	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These deviations are addressed by augmenting the model to account for decentralized flow in some microprocessor networks ( e.g. in logic networks ) .
	manualset3
173792	5	413547	7	NULL	NULL	0	NULL	logic networks	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These deviations are addressed by augmenting the model to account for decentralized flow in some microprocessor networks ( e.g. in logic networks ) .
	manualset3
173793	1	413548	7	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These differences maybe due to off-target effects of the inhibitor or PAR-4 compensation of PAR-1 deficiency .
	manualset3
173794	2	413548	7	NULL	NULL	0	NULL	 off-target effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These differences maybe due to off-target effects of the inhibitor or PAR-4 compensation of PAR-1 deficiency .
	manualset3
173795	3	413548	7	NULL	NULL	0	NULL	inhibitor	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These differences maybe due to off-target effects of the inhibitor or PAR-4 compensation of PAR-1 deficiency .
	manualset3
173796	4	413548	7	NULL	NULL	0	NULL	PAR-4 compensation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These differences maybe due to off-target effects of the inhibitor or PAR-4 compensation of PAR-1 deficiency .
	manualset3
173797	5	413548	7	NULL	NULL	0	NULL	PAR-1 deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These differences maybe due to off-target effects of the inhibitor or PAR-4 compensation of PAR-1 deficiency .
	manualset3
173798	1	413549	7	NULL	NULL	NULL	NULL	Acute tonsillopharyngitis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Acute tonsillopharyngitis is one of the most common childhood diseases .
	manualset3
173799	2	413549	7	NULL	NULL	0	NULL	childhood diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute tonsillopharyngitis is one of the most common childhood diseases .
	manualset3
173800	1	413550	7	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These differences were analyzed in relation to the function of PLA2 .
	manualset3
173801	2	413550	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These differences were analyzed in relation to the function of PLA2 .
	manualset3
173802	3	413550	7	NULL	NULL	0	NULL	function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These differences were analyzed in relation to the function of PLA2 .
	manualset3
173803	4	413550	7	NULL	NULL	0	NULL	PLA2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These differences were analyzed in relation to the function of PLA2 .
	manualset3
173804	1	413551	7	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These differences were directly related to transient differences in plasma free fluorescein concentrations , and in both cases , retinal fluorescence in diabetic rats returned to control values in conjunction with return to control levels of their plasma free fluorescein concentrations .
	manualset3
173805	2	413551	7	NULL	NULL	0	NULL	transient differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These differences were directly related to transient differences in plasma free fluorescein concentrations , and in both cases , retinal fluorescence in diabetic rats returned to control values in conjunction with return to control levels of their plasma free fluorescein concentrations .
	manualset3
173806	3	413551	7	NULL	NULL	0	NULL	plasma free fluorescein concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These differences were directly related to transient differences in plasma free fluorescein concentrations , and in both cases , retinal fluorescence in diabetic rats returned to control values in conjunction with return to control levels of their plasma free fluorescein concentrations .
	manualset3
173807	4	413551	7	NULL	NULL	0	NULL	cases	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These differences were directly related to transient differences in plasma free fluorescein concentrations , and in both cases , retinal fluorescence in diabetic rats returned to control values in conjunction with return to control levels of their plasma free fluorescein concentrations .
	manualset3
173808	5	413551	7	NULL	NULL	0	NULL	 retinal fluorescence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These differences were directly related to transient differences in plasma free fluorescein concentrations , and in both cases , retinal fluorescence in diabetic rats returned to control values in conjunction with return to control levels of their plasma free fluorescein concentrations .
	manualset3
173809	6	413551	7	NULL	NULL	0	NULL	diabetic rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These differences were directly related to transient differences in plasma free fluorescein concentrations , and in both cases , retinal fluorescence in diabetic rats returned to control values in conjunction with return to control levels of their plasma free fluorescein concentrations .
	manualset3
173810	7	413551	7	NULL	NULL	0	NULL	control values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These differences were directly related to transient differences in plasma free fluorescein concentrations , and in both cases , retinal fluorescence in diabetic rats returned to control values in conjunction with return to control levels of their plasma free fluorescein concentrations .
	manualset3
173811	8	413551	7	NULL	NULL	0	NULL	conjunction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These differences were directly related to transient differences in plasma free fluorescein concentrations , and in both cases , retinal fluorescence in diabetic rats returned to control values in conjunction with return to control levels of their plasma free fluorescein concentrations .
	manualset3
173812	9	413551	7	NULL	NULL	0	NULL	return	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These differences were directly related to transient differences in plasma free fluorescein concentrations , and in both cases , retinal fluorescence in diabetic rats returned to control values in conjunction with return to control levels of their plasma free fluorescein concentrations .
	manualset3
173813	10	413551	7	NULL	NULL	0	NULL	control levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These differences were directly related to transient differences in plasma free fluorescein concentrations , and in both cases , retinal fluorescence in diabetic rats returned to control values in conjunction with return to control levels of their plasma free fluorescein concentrations .
	manualset3
173814	11	413551	7	NULL	NULL	0	NULL	plasma free fluorescein concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These differences were directly related to transient differences in plasma free fluorescein concentrations , and in both cases , retinal fluorescence in diabetic rats returned to control values in conjunction with return to control levels of their plasma free fluorescein concentrations .
	manualset3
173815	1	413552	7	NULL	NULL	0	NULL	phonetic targets	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These different phonetic targets were predicted to result in different enhancement patterns in clear speech : Younger speakers were predicted to enhance F0 differences , whereas older speakers were predicted to enhance VOT differences in clear speech .
	manualset3
173816	2	413552	7	NULL	NULL	0	NULL	different enhancement patterns	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These different phonetic targets were predicted to result in different enhancement patterns in clear speech : Younger speakers were predicted to enhance F0 differences , whereas older speakers were predicted to enhance VOT differences in clear speech .
	manualset3
173817	3	413552	7	NULL	NULL	NULL	NULL	clear speech	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These different phonetic targets were predicted to result in different enhancement patterns in clear speech : Younger speakers were predicted to enhance F0 differences , whereas older speakers were predicted to enhance VOT differences in clear speech .
	manualset3
173818	4	413552	7	NULL	NULL	0	NULL	Younger speakers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These different phonetic targets were predicted to result in different enhancement patterns in clear speech : Younger speakers were predicted to enhance F0 differences , whereas older speakers were predicted to enhance VOT differences in clear speech .
	manualset3
173819	5	413552	7	NULL	NULL	0	NULL	F0 differences	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These different phonetic targets were predicted to result in different enhancement patterns in clear speech : Younger speakers were predicted to enhance F0 differences , whereas older speakers were predicted to enhance VOT differences in clear speech .
	manualset3
173820	6	413552	7	NULL	NULL	0	NULL	older speakers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These different phonetic targets were predicted to result in different enhancement patterns in clear speech : Younger speakers were predicted to enhance F0 differences , whereas older speakers were predicted to enhance VOT differences in clear speech .
	manualset3
173821	7	413552	7	NULL	NULL	0	NULL	 VOT differences	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These different phonetic targets were predicted to result in different enhancement patterns in clear speech : Younger speakers were predicted to enhance F0 differences , whereas older speakers were predicted to enhance VOT differences in clear speech .
	manualset3
173822	8	413552	7	NULL	NULL	0	NULL	clear speech	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These different phonetic targets were predicted to result in different enhancement patterns in clear speech : Younger speakers were predicted to enhance F0 differences , whereas older speakers were predicted to enhance VOT differences in clear speech .
	manualset3
173830	1	413553	7	NULL	NULL	0	NULL	diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These diseases , especially dermatomyositis , have a well-known association with a wide variety of neoplasms including lung , breast , ovary and colon cancers .
	manualset3
173833	2	413553	7	NULL	NULL	0	NULL	dermatomyositis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These diseases , especially dermatomyositis , have a well-known association with a wide variety of neoplasms including lung , breast , ovary and colon cancers .
	manualset3
173834	3	413553	7	NULL	NULL	NULL	NULL	association	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These diseases , especially dermatomyositis , have a well-known association with a wide variety of neoplasms including lung , breast , ovary and colon cancers .
	manualset3
173835	4	413553	7	NULL	NULL	0	NULL	neoplasms	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These diseases , especially dermatomyositis , have a well-known association with a wide variety of neoplasms including lung , breast , ovary and colon cancers .
	manualset3
173836	5	413553	7	NULL	NULL	0	NULL	 lung cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These diseases , especially dermatomyositis , have a well-known association with a wide variety of neoplasms including lung , breast , ovary and colon cancers .
	manualset3
173837	6	413553	7	NULL	NULL	0	NULL	 breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These diseases , especially dermatomyositis , have a well-known association with a wide variety of neoplasms including lung , breast , ovary and colon cancers .
	manualset3
173840	7	413553	7	NULL	NULL	0	NULL	 ovary cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These diseases , especially dermatomyositis , have a well-known association with a wide variety of neoplasms including lung , breast , ovary and colon cancers .
	manualset3
173841	8	413553	7	NULL	NULL	0	NULL	colon cancers	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These diseases , especially dermatomyositis , have a well-known association with a wide variety of neoplasms including lung , breast , ovary and colon cancers .
	manualset3
173852	1	413554	7	NULL	NULL	0	NULL	effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects of CSF were blocked by naloxone administration and were observed only if injecting CSF which was preliminarily treated with protease inhibitors .
	manualset3
173853	2	413554	7	NULL	NULL	0	NULL	CSF	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects of CSF were blocked by naloxone administration and were observed only if injecting CSF which was preliminarily treated with protease inhibitors .
	manualset3
173854	3	413554	7	NULL	NULL	0	NULL	naloxone administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects of CSF were blocked by naloxone administration and were observed only if injecting CSF which was preliminarily treated with protease inhibitors .
	manualset3
173855	4	413554	7	NULL	NULL	0	NULL	CSF	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects of CSF were blocked by naloxone administration and were observed only if injecting CSF which was preliminarily treated with protease inhibitors .
	manualset3
173856	5	413554	7	NULL	NULL	0	NULL	protease inhibitors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects of CSF were blocked by naloxone administration and were observed only if injecting CSF which was preliminarily treated with protease inhibitors .
	manualset3
173947	1	413555	7	NULL	NULL	0	NULL	( 3H ) AII 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3H ) AII was not degraded by the microsomes but 125I-labelled AII was degraded .
	manualset3
173948	2	413555	7	NULL	NULL	0	NULL	microsomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3H ) AII was not degraded by the microsomes but 125I-labelled AII was degraded .
	manualset3
173949	3	413555	7	NULL	NULL	0	NULL	125I-labelled AII	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3H ) AII was not degraded by the microsomes but 125I-labelled AII was degraded .
	manualset3
173966	1	413556	7	NULL	NULL	0	NULL	Comparative cytogenetic study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative cytogenetic study of 7 types of mammary cancer ) .
	manualset3
173967	2	413556	7	NULL	NULL	0	NULL	 7 types	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative cytogenetic study of 7 types of mammary cancer ) .
	manualset3
173968	3	413556	7	NULL	NULL	0	NULL	mammary cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative cytogenetic study of 7 types of mammary cancer ) .
	manualset3
173969	1	413557	7	NULL	NULL	0	NULL	Acute weight gain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute weight gain and diastolic dysfunction as a potent risk complex for post stem cell transplant atrial fibrillation .
	manualset3
173970	2	413557	7	NULL	NULL	0	NULL	diastolic dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute weight gain and diastolic dysfunction as a potent risk complex for post stem cell transplant atrial fibrillation .
	manualset3
173971	3	413557	7	NULL	NULL	0	NULL	potent risk complex	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute weight gain and diastolic dysfunction as a potent risk complex for post stem cell transplant atrial fibrillation .
	manualset3
173972	4	413557	7	NULL	NULL	0	NULL	post stem cell transplant atrial fibrillation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute weight gain and diastolic dysfunction as a potent risk complex for post stem cell transplant atrial fibrillation .
	manualset3
173973	1	413558	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects of lactate on the Na + channel might alter electrophysiological properties during myocardial ischemia and could protect the heart from ischemia-induced conduction abnormalities or , alternatively , could lead to arrhythmias .
	manualset3
173974	2	413558	7	NULL	NULL	0	NULL	 lactate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects of lactate on the Na + channel might alter electrophysiological properties during myocardial ischemia and could protect the heart from ischemia-induced conduction abnormalities or , alternatively , could lead to arrhythmias .
	manualset3
173975	3	413558	7	NULL	NULL	0	NULL	Na + channel	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects of lactate on the Na + channel might alter electrophysiological properties during myocardial ischemia and could protect the heart from ischemia-induced conduction abnormalities or , alternatively , could lead to arrhythmias .
	manualset3
173976	4	413558	7	NULL	NULL	0	NULL	electrophysiological properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects of lactate on the Na + channel might alter electrophysiological properties during myocardial ischemia and could protect the heart from ischemia-induced conduction abnormalities or , alternatively , could lead to arrhythmias .
	manualset3
173977	5	413558	7	NULL	NULL	0	NULL	myocardial ischemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects of lactate on the Na + channel might alter electrophysiological properties during myocardial ischemia and could protect the heart from ischemia-induced conduction abnormalities or , alternatively , could lead to arrhythmias .
	manualset3
173978	6	413558	7	NULL	NULL	0	NULL	heart	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects of lactate on the Na + channel might alter electrophysiological properties during myocardial ischemia and could protect the heart from ischemia-induced conduction abnormalities or , alternatively , could lead to arrhythmias .
	manualset3
173979	7	413558	7	NULL	NULL	0	NULL	ischemia-induced conduction abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects of lactate on the Na + channel might alter electrophysiological properties during myocardial ischemia and could protect the heart from ischemia-induced conduction abnormalities or , alternatively , could lead to arrhythmias .
	manualset3
173980	8	413558	7	NULL	NULL	0	NULL	arrhythmias	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects of lactate on the Na + channel might alter electrophysiological properties during myocardial ischemia and could protect the heart from ischemia-induced conduction abnormalities or , alternatively , could lead to arrhythmias .
	manualset3
173981	1	413559	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects of the derivatives were generally more markedly expressed than those of trapidil .
	manualset3
173982	2	413559	7	NULL	NULL	0	NULL	derivatives	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects of the derivatives were generally more markedly expressed than those of trapidil .
	manualset3
173983	3	413559	7	NULL	NULL	0	NULL	trapidil	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects of the derivatives were generally more markedly expressed than those of trapidil .
	manualset3
173984	1	413560	7	NULL	NULL	0	NULL	effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects on cell proliferation were not due to the LPL cytolysis as viability and cell membrane integrity were not altered .
	manualset3
173985	2	413560	7	NULL	NULL	0	NULL	cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects on cell proliferation were not due to the LPL cytolysis as viability and cell membrane integrity were not altered .
	manualset3
173986	3	413560	7	NULL	NULL	0	NULL	 LPL cytolysis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects on cell proliferation were not due to the LPL cytolysis as viability and cell membrane integrity were not altered .
	manualset3
173987	4	413560	7	NULL	NULL	0	NULL	viability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects on cell proliferation were not due to the LPL cytolysis as viability and cell membrane integrity were not altered .
	manualset3
173988	5	413560	7	NULL	NULL	0	NULL	cell membrane integrity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects on cell proliferation were not due to the LPL cytolysis as viability and cell membrane integrity were not altered .
	manualset3
173989	1	413561	7	NULL	NULL	0	NULL	effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects seem to be modulated by changes in chromatin structure .
	manualset3
173991	2	413561	7	NULL	NULL	0	NULL	changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects seem to be modulated by changes in chromatin structure .
	manualset3
173992	3	413561	7	NULL	NULL	0	NULL	chromatin structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects seem to be modulated by changes in chromatin structure .
	manualset3
174024	1	413562	7	NULL	NULL	0	NULL	effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects were attenuated by prior administration of cimetidine .
	manualset3
174025	2	413562	7	NULL	NULL	0	NULL	 administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects were attenuated by prior administration of cimetidine .
	manualset3
174026	3	413562	7	NULL	NULL	0	NULL	cimetidine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects were attenuated by prior administration of cimetidine .
	manualset3
174027	1	413563	7	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects were blocked by the A ( 2A ) receptor antagonist 4 - ( 2 - ( 7-amino-2 - ( 2-furyl ) ( 1 , 2 , 4-triazolo ( 2 , 3-a ) ( 1 , 3 , 5 ) triazin-5-ylamino ) ethyl ) phenol ( ZM-241385 ) .
	manualset3
174028	2	413563	7	NULL	NULL	0	NULL	 A ( 2A ) receptor antagonist	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects were blocked by the A ( 2A ) receptor antagonist 4 - ( 2 - ( 7-amino-2 - ( 2-furyl ) ( 1 , 2 , 4-triazolo ( 2 , 3-a ) ( 1 , 3 , 5 ) triazin-5-ylamino ) ethyl ) phenol ( ZM-241385 ) .
	manualset3
174029	3	413563	7	NULL	NULL	0	NULL	4 - ( 2 - ( 7-amino-2 - ( 2-furyl ) ( 1 , 2 , 4-triazolo ( 2 , 3-a ) ( 1 , 3 , 5 ) triazin-5-ylamino ) ethyl ) phenol ( ZM-241385 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects were blocked by the A ( 2A ) receptor antagonist 4 - ( 2 - ( 7-amino-2 - ( 2-furyl ) ( 1 , 2 , 4-triazolo ( 2 , 3-a ) ( 1 , 3 , 5 ) triazin-5-ylamino ) ethyl ) phenol ( ZM-241385 ) .
	manualset3
174030	1	413564	7	NULL	NULL	NULL	NULL	 effects 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These effects were lowered when the transmembrane delta pH was dissipated , which indicates that the neutral form of the drug is implicated in the uncoupling mechanism .
	manualset3
174031	2	413564	7	NULL	NULL	0	NULL	transmembrane delta pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects were lowered when the transmembrane delta pH was dissipated , which indicates that the neutral form of the drug is implicated in the uncoupling mechanism .
	manualset3
174032	3	413564	7	NULL	NULL	0	NULL	 neutral form	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects were lowered when the transmembrane delta pH was dissipated , which indicates that the neutral form of the drug is implicated in the uncoupling mechanism .
	manualset3
174033	4	413564	7	NULL	NULL	0	NULL	drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects were lowered when the transmembrane delta pH was dissipated , which indicates that the neutral form of the drug is implicated in the uncoupling mechanism .
	manualset3
174034	5	413564	7	NULL	NULL	0	NULL	uncoupling mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These effects were lowered when the transmembrane delta pH was dissipated , which indicates that the neutral form of the drug is implicated in the uncoupling mechanism .
	manualset3
174035	1	413565	7	NULL	NULL	0	NULL	ephrinB2-dependent events	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These ephrinB2-dependent events result in enhanced NMDA receptor-dependent gene expression .
	manualset3
174036	2	413565	7	NULL	NULL	0	NULL	NMDA receptor-dependent gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These ephrinB2-dependent events result in enhanced NMDA receptor-dependent gene expression .
	manualset3
174037	1	413566	7	NULL	NULL	0	NULL	Acyclovir ( 9 - ( 2-hydroxyethoxymethyl ) guanine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Acyclovir ( 9 - ( 2-hydroxyethoxymethyl ) guanine , ZoviraxTM ) is a selective antiviral agent with indications for the treatment of the herpes virus group of injections .
	manualset3
174038	2	413566	7	NULL	NULL	0	NULL	ZoviraxTM	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Acyclovir ( 9 - ( 2-hydroxyethoxymethyl ) guanine , ZoviraxTM ) is a selective antiviral agent with indications for the treatment of the herpes virus group of injections .
	manualset3
174039	3	413566	7	NULL	NULL	0	NULL	selective antiviral agent	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Acyclovir ( 9 - ( 2-hydroxyethoxymethyl ) guanine , ZoviraxTM ) is a selective antiviral agent with indications for the treatment of the herpes virus group of injections .
	manualset3
174040	4	413566	7	NULL	NULL	0	NULL	indications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acyclovir ( 9 - ( 2-hydroxyethoxymethyl ) guanine , ZoviraxTM ) is a selective antiviral agent with indications for the treatment of the herpes virus group of injections .
	manualset3
174041	5	413566	7	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Acyclovir ( 9 - ( 2-hydroxyethoxymethyl ) guanine , ZoviraxTM ) is a selective antiviral agent with indications for the treatment of the herpes virus group of injections .
	manualset3
174042	6	413566	7	NULL	NULL	NULL	NULL	herpes virus group	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Acyclovir ( 9 - ( 2-hydroxyethoxymethyl ) guanine , ZoviraxTM ) is a selective antiviral agent with indications for the treatment of the herpes virus group of injections .
	manualset3
174043	7	413566	7	NULL	NULL	0	NULL	 injections	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Acyclovir ( 9 - ( 2-hydroxyethoxymethyl ) guanine , ZoviraxTM ) is a selective antiviral agent with indications for the treatment of the herpes virus group of injections .
	manualset3
174107	1	413567	7	NULL	NULL	NULL	NULL	examples	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These examples , representing the areas of photovoltaics , microelectronics , microelectromechanics , photocatalysis , corrosion prevention and even biomedicine should be regarded as appetizers paving the way for further studies to be performed .
	manualset3
174108	2	413567	7	NULL	NULL	0	NULL	areas	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These examples , representing the areas of photovoltaics , microelectronics , microelectromechanics , photocatalysis , corrosion prevention and even biomedicine should be regarded as appetizers paving the way for further studies to be performed .
	manualset3
174109	3	413567	7	NULL	NULL	0	NULL	photovoltaics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These examples , representing the areas of photovoltaics , microelectronics , microelectromechanics , photocatalysis , corrosion prevention and even biomedicine should be regarded as appetizers paving the way for further studies to be performed .
	manualset3
174110	4	413567	7	NULL	NULL	0	NULL	 microelectronics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These examples , representing the areas of photovoltaics , microelectronics , microelectromechanics , photocatalysis , corrosion prevention and even biomedicine should be regarded as appetizers paving the way for further studies to be performed .
	manualset3
174111	5	413567	7	NULL	NULL	0	NULL	microelectromechanics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These examples , representing the areas of photovoltaics , microelectronics , microelectromechanics , photocatalysis , corrosion prevention and even biomedicine should be regarded as appetizers paving the way for further studies to be performed .
	manualset3
174112	6	413567	7	NULL	NULL	0	NULL	photocatalysis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These examples , representing the areas of photovoltaics , microelectronics , microelectromechanics , photocatalysis , corrosion prevention and even biomedicine should be regarded as appetizers paving the way for further studies to be performed .
	manualset3
174113	7	413567	7	NULL	NULL	0	NULL	corrosion prevention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These examples , representing the areas of photovoltaics , microelectronics , microelectromechanics , photocatalysis , corrosion prevention and even biomedicine should be regarded as appetizers paving the way for further studies to be performed .
	manualset3
174114	8	413567	7	NULL	NULL	0	NULL	biomedicine	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These examples , representing the areas of photovoltaics , microelectronics , microelectromechanics , photocatalysis , corrosion prevention and even biomedicine should be regarded as appetizers paving the way for further studies to be performed .
	manualset3
174115	9	413567	7	NULL	NULL	NULL	NULL	appetizers 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These examples , representing the areas of photovoltaics , microelectronics , microelectromechanics , photocatalysis , corrosion prevention and even biomedicine should be regarded as appetizers paving the way for further studies to be performed .
	manualset3
174116	10	413567	7	NULL	NULL	0	NULL	way	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These examples , representing the areas of photovoltaics , microelectronics , microelectromechanics , photocatalysis , corrosion prevention and even biomedicine should be regarded as appetizers paving the way for further studies to be performed .
	manualset3
174566	11	413567	7	NULL	NULL	0	NULL	 studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These examples , representing the areas of photovoltaics , microelectronics , microelectromechanics , photocatalysis , corrosion prevention and even biomedicine should be regarded as appetizers paving the way for further studies to be performed .
	manualset3
174117	1	413568	7	NULL	NULL	0	NULL	 examples	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These examples accentuate the need for continued participation of human biologists in the study of growth and development and the care of children .
	manualset3
174118	2	413568	7	NULL	NULL	0	NULL	need	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These examples accentuate the need for continued participation of human biologists in the study of growth and development and the care of children .
	manualset3
174119	3	413568	7	NULL	NULL	0	NULL	continued participation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These examples accentuate the need for continued participation of human biologists in the study of growth and development and the care of children .
	manualset3
174120	4	413568	7	NULL	NULL	0	NULL	human biologists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These examples accentuate the need for continued participation of human biologists in the study of growth and development and the care of children .
	manualset3
174121	5	413568	7	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These examples accentuate the need for continued participation of human biologists in the study of growth and development and the care of children .
	manualset3
174122	6	413568	7	NULL	NULL	0	NULL	growth	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These examples accentuate the need for continued participation of human biologists in the study of growth and development and the care of children .
	manualset3
174123	7	413568	7	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These examples accentuate the need for continued participation of human biologists in the study of growth and development and the care of children .
	manualset3
174124	8	413568	7	NULL	NULL	0	NULL	 care	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These examples accentuate the need for continued participation of human biologists in the study of growth and development and the care of children .
	manualset3
174125	9	413568	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These examples accentuate the need for continued participation of human biologists in the study of growth and development and the care of children .
	manualset3
174126	1	413569	7	NULL	NULL	0	NULL	experimental data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These experimental data suggest that inhaled NO significantly exacerbated acute lung injury induced by PMA in rats .
	manualset3
174127	2	413569	7	NULL	NULL	0	NULL	inhaled NO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These experimental data suggest that inhaled NO significantly exacerbated acute lung injury induced by PMA in rats .
	manualset3
174128	3	413569	7	NULL	NULL	0	NULL	acute lung injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These experimental data suggest that inhaled NO significantly exacerbated acute lung injury induced by PMA in rats .
	manualset3
174129	4	413569	7	NULL	NULL	0	NULL	PMA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These experimental data suggest that inhaled NO significantly exacerbated acute lung injury induced by PMA in rats .
	manualset3
174130	5	413569	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These experimental data suggest that inhaled NO significantly exacerbated acute lung injury induced by PMA in rats .
	manualset3
174131	1	413570	7	NULL	NULL	NULL	NULL	experiments	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These experiments also provide the first direct identification of surface micelles on water , and the first identification of such large-size domains using GISAXS .
	manualset3
174132	2	413570	7	NULL	NULL	NULL	NULL	first direct identification	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These experiments also provide the first direct identification of surface micelles on water , and the first identification of such large-size domains using GISAXS .
	manualset3
174133	3	413570	7	NULL	NULL	0	NULL	surface micelles 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These experiments also provide the first direct identification of surface micelles on water , and the first identification of such large-size domains using GISAXS .
	manualset3
174134	4	413570	7	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These experiments also provide the first direct identification of surface micelles on water , and the first identification of such large-size domains using GISAXS .
	manualset3
174135	5	413570	7	NULL	NULL	0	NULL	first identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These experiments also provide the first direct identification of surface micelles on water , and the first identification of such large-size domains using GISAXS .
	manualset3
174136	6	413570	7	NULL	NULL	0	NULL	large-size domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These experiments also provide the first direct identification of surface micelles on water , and the first identification of such large-size domains using GISAXS .
	manualset3
174137	7	413570	7	NULL	NULL	0	NULL	 GISAXS	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These experiments also provide the first direct identification of surface micelles on water , and the first identification of such large-size domains using GISAXS .
	manualset3
174138	1	413571	7	NULL	NULL	0	NULL	experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These experiments strongly indicate that zingerone treatment exerts a beneficial efficacy by suppressing both oxidative stress and age-related inflammation through the modulation of several key pro-inflammatory genes and transcription factors .
	manualset3
174578	2	413571	7	NULL	NULL	0	NULL	zingerone treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These experiments strongly indicate that zingerone treatment exerts a beneficial efficacy by suppressing both oxidative stress and age-related inflammation through the modulation of several key pro-inflammatory genes and transcription factors .
	manualset3
174579	3	413571	7	NULL	NULL	0	NULL	beneficial efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These experiments strongly indicate that zingerone treatment exerts a beneficial efficacy by suppressing both oxidative stress and age-related inflammation through the modulation of several key pro-inflammatory genes and transcription factors .
	manualset3
174580	4	413571	7	NULL	NULL	0	NULL	oxidative stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These experiments strongly indicate that zingerone treatment exerts a beneficial efficacy by suppressing both oxidative stress and age-related inflammation through the modulation of several key pro-inflammatory genes and transcription factors .
	manualset3
174581	5	413571	7	NULL	NULL	0	NULL	age-related inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These experiments strongly indicate that zingerone treatment exerts a beneficial efficacy by suppressing both oxidative stress and age-related inflammation through the modulation of several key pro-inflammatory genes and transcription factors .
	manualset3
174582	6	413571	7	NULL	NULL	0	NULL	modulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These experiments strongly indicate that zingerone treatment exerts a beneficial efficacy by suppressing both oxidative stress and age-related inflammation through the modulation of several key pro-inflammatory genes and transcription factors .
	manualset3
174584	7	413571	7	NULL	NULL	0	NULL	pro-inflammatory genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These experiments strongly indicate that zingerone treatment exerts a beneficial efficacy by suppressing both oxidative stress and age-related inflammation through the modulation of several key pro-inflammatory genes and transcription factors .
	manualset3
174587	8	413571	7	NULL	NULL	NULL	NULL	 transcription factors	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These experiments strongly indicate that zingerone treatment exerts a beneficial efficacy by suppressing both oxidative stress and age-related inflammation through the modulation of several key pro-inflammatory genes and transcription factors .
	manualset3
174605	1	413572	7	NULL	NULL	0	NULL	extended-temperature-range evaluations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These extended-temperature-range evaluations , given as three-parameter fits , are as follows : kOH + n-heptane ) 2.059 x 10 ( -15 ) T1 .401 exp ( 33 K / T ) cm3 molecule-1 s-1 ( 241-1287 K ) kOH +2 , 2 , 3 , 3 - TMB ) 6.835 x 10 ( -17 ) T1 .886 exp ( -365 K / T ) cm3 molecule-1 s-1 ( 290-1180 K ) kOH + n-pentane ) 2.495 x 10 ( -16 ) T1 .649 exp ( 80 K/T ) cm3 molecule-1 s-1 ( 224-1308 K ) kOH + n-hexane ) 3.959 x 10 ( -18 ) T2 .218 exp ( 443 K/T ) cm3 molecule-1 s-1 ( 292-1299 K ) kOH +2 , 3 - DMB ) 2.287 x 10 ( -17 ) T1 .958 exp ( 365 K / T ) cm3 molecule-1 s-1 ( 220-1292 K ) .
	manualset3
174608	2	413572	7	NULL	NULL	0	NULL	 three-parameter fits	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These extended-temperature-range evaluations , given as three-parameter fits , are as follows : kOH + n-heptane ) 2.059 x 10 ( -15 ) T1 .401 exp ( 33 K / T ) cm3 molecule-1 s-1 ( 241-1287 K ) kOH +2 , 2 , 3 , 3 - TMB ) 6.835 x 10 ( -17 ) T1 .886 exp ( -365 K / T ) cm3 molecule-1 s-1 ( 290-1180 K ) kOH + n-pentane ) 2.495 x 10 ( -16 ) T1 .649 exp ( 80 K/T ) cm3 molecule-1 s-1 ( 224-1308 K ) kOH + n-hexane ) 3.959 x 10 ( -18 ) T2 .218 exp ( 443 K/T ) cm3 molecule-1 s-1 ( 292-1299 K ) kOH +2 , 3 - DMB ) 2.287 x 10 ( -17 ) T1 .958 exp ( 365 K / T ) cm3 molecule-1 s-1 ( 220-1292 K ) .
	manualset3
174622	3	413572	7	NULL	NULL	0	NULL	kOH + n-heptane ) 2.059 x 10 ( -15 ) T1 .401 exp ( 33 K / T ) cm3 molecule-1 s-1 ( 241-1287 K )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These extended-temperature-range evaluations , given as three-parameter fits , are as follows : kOH + n-heptane ) 2.059 x 10 ( -15 ) T1 .401 exp ( 33 K / T ) cm3 molecule-1 s-1 ( 241-1287 K ) kOH +2 , 2 , 3 , 3 - TMB ) 6.835 x 10 ( -17 ) T1 .886 exp ( -365 K / T ) cm3 molecule-1 s-1 ( 290-1180 K ) kOH + n-pentane ) 2.495 x 10 ( -16 ) T1 .649 exp ( 80 K/T ) cm3 molecule-1 s-1 ( 224-1308 K ) kOH + n-hexane ) 3.959 x 10 ( -18 ) T2 .218 exp ( 443 K/T ) cm3 molecule-1 s-1 ( 292-1299 K ) kOH +2 , 3 - DMB ) 2.287 x 10 ( -17 ) T1 .958 exp ( 365 K / T ) cm3 molecule-1 s-1 ( 220-1292 K ) .
	manualset3
174625	4	413572	7	NULL	NULL	0	NULL	kOH +2 , 2 , 3 , 3 - TMB ) 6.835 x 10 ( -17 ) T1 .886 exp ( -365 K / T ) cm3 molecule-1 s-1 ( 290-1180 K ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These extended-temperature-range evaluations , given as three-parameter fits , are as follows : kOH + n-heptane ) 2.059 x 10 ( -15 ) T1 .401 exp ( 33 K / T ) cm3 molecule-1 s-1 ( 241-1287 K ) kOH +2 , 2 , 3 , 3 - TMB ) 6.835 x 10 ( -17 ) T1 .886 exp ( -365 K / T ) cm3 molecule-1 s-1 ( 290-1180 K ) kOH + n-pentane ) 2.495 x 10 ( -16 ) T1 .649 exp ( 80 K/T ) cm3 molecule-1 s-1 ( 224-1308 K ) kOH + n-hexane ) 3.959 x 10 ( -18 ) T2 .218 exp ( 443 K/T ) cm3 molecule-1 s-1 ( 292-1299 K ) kOH +2 , 3 - DMB ) 2.287 x 10 ( -17 ) T1 .958 exp ( 365 K / T ) cm3 molecule-1 s-1 ( 220-1292 K ) .
	manualset3
174627	5	413572	7	NULL	NULL	0	NULL	kOH + n-pentane ) 2.495 x 10 ( -16 ) T1 .649 exp ( 80 K/T ) cm3 molecule-1 s-1 ( 224-1308 K ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These extended-temperature-range evaluations , given as three-parameter fits , are as follows : kOH + n-heptane ) 2.059 x 10 ( -15 ) T1 .401 exp ( 33 K / T ) cm3 molecule-1 s-1 ( 241-1287 K ) kOH +2 , 2 , 3 , 3 - TMB ) 6.835 x 10 ( -17 ) T1 .886 exp ( -365 K / T ) cm3 molecule-1 s-1 ( 290-1180 K ) kOH + n-pentane ) 2.495 x 10 ( -16 ) T1 .649 exp ( 80 K/T ) cm3 molecule-1 s-1 ( 224-1308 K ) kOH + n-hexane ) 3.959 x 10 ( -18 ) T2 .218 exp ( 443 K/T ) cm3 molecule-1 s-1 ( 292-1299 K ) kOH +2 , 3 - DMB ) 2.287 x 10 ( -17 ) T1 .958 exp ( 365 K / T ) cm3 molecule-1 s-1 ( 220-1292 K ) .
	manualset3
174628	6	413572	7	NULL	NULL	0	NULL	kOH + n-hexane ) 3.959 x 10 ( -18 ) T2 .218 exp ( 443 K/T ) cm3 molecule-1 s-1 ( 292-1299 K )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These extended-temperature-range evaluations , given as three-parameter fits , are as follows : kOH + n-heptane ) 2.059 x 10 ( -15 ) T1 .401 exp ( 33 K / T ) cm3 molecule-1 s-1 ( 241-1287 K ) kOH +2 , 2 , 3 , 3 - TMB ) 6.835 x 10 ( -17 ) T1 .886 exp ( -365 K / T ) cm3 molecule-1 s-1 ( 290-1180 K ) kOH + n-pentane ) 2.495 x 10 ( -16 ) T1 .649 exp ( 80 K/T ) cm3 molecule-1 s-1 ( 224-1308 K ) kOH + n-hexane ) 3.959 x 10 ( -18 ) T2 .218 exp ( 443 K/T ) cm3 molecule-1 s-1 ( 292-1299 K ) kOH +2 , 3 - DMB ) 2.287 x 10 ( -17 ) T1 .958 exp ( 365 K / T ) cm3 molecule-1 s-1 ( 220-1292 K ) .
	manualset3
174630	7	413572	7	NULL	NULL	0	NULL	kOH +2 , 3 - DMB ) 2.287 x 10 ( -17 ) T1 .958 exp ( 365 K / T ) cm3 molecule-1 s-1 ( 220-1292 K )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These extended-temperature-range evaluations , given as three-parameter fits , are as follows : kOH + n-heptane ) 2.059 x 10 ( -15 ) T1 .401 exp ( 33 K / T ) cm3 molecule-1 s-1 ( 241-1287 K ) kOH +2 , 2 , 3 , 3 - TMB ) 6.835 x 10 ( -17 ) T1 .886 exp ( -365 K / T ) cm3 molecule-1 s-1 ( 290-1180 K ) kOH + n-pentane ) 2.495 x 10 ( -16 ) T1 .649 exp ( 80 K/T ) cm3 molecule-1 s-1 ( 224-1308 K ) kOH + n-hexane ) 3.959 x 10 ( -18 ) T2 .218 exp ( 443 K/T ) cm3 molecule-1 s-1 ( 292-1299 K ) kOH +2 , 3 - DMB ) 2.287 x 10 ( -17 ) T1 .958 exp ( 365 K / T ) cm3 molecule-1 s-1 ( 220-1292 K ) .
	manualset3
174641	1	413573	7	NULL	NULL	NULL	NULL	Ad.mda-7	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ad.mda-7 reduced the proliferation of rodent and human glioma cells in MTT assays and in colony formation assays .
	manualset3
174651	2	413573	7	NULL	NULL	0	NULL	proliferation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ad.mda-7 reduced the proliferation of rodent and human glioma cells in MTT assays and in colony formation assays .
	manualset3
174652	3	413573	7	NULL	NULL	NULL	NULL	rodent glioma cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ad.mda-7 reduced the proliferation of rodent and human glioma cells in MTT assays and in colony formation assays .
	manualset3
174653	4	413573	7	NULL	NULL	0	NULL	human glioma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Ad.mda-7 reduced the proliferation of rodent and human glioma cells in MTT assays and in colony formation assays .
	manualset3
174654	5	413573	7	NULL	NULL	0	NULL	MTT assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ad.mda-7 reduced the proliferation of rodent and human glioma cells in MTT assays and in colony formation assays .
	manualset3
174655	6	413573	7	NULL	NULL	0	NULL	colony formation assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ad.mda-7 reduced the proliferation of rodent and human glioma cells in MTT assays and in colony formation assays .
	manualset3
174707	1	413574	7	NULL	NULL	0	NULL	 features	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These features do not seem to be casual , but they obey a general principle : Cations recognize themselves in spite of being embedded in an oxygen bulk .
	manualset3
174712	3	413574	7	NULL	NULL	0	NULL	general principle	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These features do not seem to be casual , but they obey a general principle : Cations recognize themselves in spite of being embedded in an oxygen bulk .
	manualset3
174713	4	413574	7	NULL	NULL	0	NULL	Cations	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	These features do not seem to be casual , but they obey a general principle : Cations recognize themselves in spite of being embedded in an oxygen bulk .
	manualset3
174715	5	413574	7	NULL	NULL	0	NULL	oxygen bulk	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These features do not seem to be casual , but they obey a general principle : Cations recognize themselves in spite of being embedded in an oxygen bulk .
	manualset3
174726	1	413575	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings 1 ) suggest that matched reductions of frontal gray matter weight and perfusion occur in FLD and 2 ) support the use of rCBF in distinguishing FLD from AD and severe depression .
	manualset3
174728	2	413575	7	NULL	NULL	0	NULL	matched reductions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings 1 ) suggest that matched reductions of frontal gray matter weight and perfusion occur in FLD and 2 ) support the use of rCBF in distinguishing FLD from AD and severe depression .
	manualset3
174729	3	413575	7	NULL	NULL	0	NULL	frontal gray matter weight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings 1 ) suggest that matched reductions of frontal gray matter weight and perfusion occur in FLD and 2 ) support the use of rCBF in distinguishing FLD from AD and severe depression .
	manualset3
174730	4	413575	7	NULL	NULL	NULL	NULL	frontal gray matter perfusion	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings 1 ) suggest that matched reductions of frontal gray matter weight and perfusion occur in FLD and 2 ) support the use of rCBF in distinguishing FLD from AD and severe depression .
	manualset3
174731	5	413575	7	NULL	NULL	0	NULL	FLD	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings 1 ) suggest that matched reductions of frontal gray matter weight and perfusion occur in FLD and 2 ) support the use of rCBF in distinguishing FLD from AD and severe depression .
	manualset3
174732	6	413575	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings 1 ) suggest that matched reductions of frontal gray matter weight and perfusion occur in FLD and 2 ) support the use of rCBF in distinguishing FLD from AD and severe depression .
	manualset3
174733	7	413575	7	NULL	NULL	0	NULL	rCBF	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings 1 ) suggest that matched reductions of frontal gray matter weight and perfusion occur in FLD and 2 ) support the use of rCBF in distinguishing FLD from AD and severe depression .
	manualset3
174734	8	413575	7	NULL	NULL	0	NULL	FLD	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings 1 ) suggest that matched reductions of frontal gray matter weight and perfusion occur in FLD and 2 ) support the use of rCBF in distinguishing FLD from AD and severe depression .
	manualset3
174735	9	413575	7	NULL	NULL	0	NULL	AD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings 1 ) suggest that matched reductions of frontal gray matter weight and perfusion occur in FLD and 2 ) support the use of rCBF in distinguishing FLD from AD and severe depression .
	manualset3
174736	10	413575	7	NULL	NULL	0	NULL	severe depression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings 1 ) suggest that matched reductions of frontal gray matter weight and perfusion occur in FLD and 2 ) support the use of rCBF in distinguishing FLD from AD and severe depression .
	manualset3
174737	1	413576	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings add an important dimension to our understanding of the underlying processes of hearing maturation .
	manualset3
174738	2	413576	7	NULL	NULL	0	NULL	 dimension	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings add an important dimension to our understanding of the underlying processes of hearing maturation .
	manualset3
174739	3	413576	7	NULL	NULL	NULL	NULL	understanding	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings add an important dimension to our understanding of the underlying processes of hearing maturation .
	manualset3
174740	4	413576	7	NULL	NULL	0	NULL	underlying processes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings add an important dimension to our understanding of the underlying processes of hearing maturation .
	manualset3
174746	5	413576	7	NULL	NULL	0	NULL	hearing maturation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings add an important dimension to our understanding of the underlying processes of hearing maturation .
	manualset3
174749	1	413577	7	NULL	NULL	0	NULL	findings 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings add to the limited literature on CPOE in community hospitals .
	manualset3
174751	2	413577	7	NULL	NULL	0	NULL	 limited literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings add to the limited literature on CPOE in community hospitals .
	manualset3
174755	3	413577	7	NULL	NULL	0	NULL	CPOE	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings add to the limited literature on CPOE in community hospitals .
	manualset3
174756	4	413577	7	NULL	NULL	0	NULL	community hospitals	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings add to the limited literature on CPOE in community hospitals .
	manualset3
174757	1	413578	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings advance our understanding of fruit body development .
	manualset3
174758	2	413578	7	NULL	NULL	NULL	NULL	understanding	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings advance our understanding of fruit body development .
	manualset3
174759	3	413578	7	NULL	NULL	0	NULL	fruit body development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings advance our understanding of fruit body development .
	manualset3
174760	1	413579	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings appear to be different than those reported for inactivation of other Atg4 homologs , suggesting that these homologs have tissue-specific functions beyond redundancy .
	manualset3
174761	2	413579	7	NULL	NULL	0	NULL	inactivation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings appear to be different than those reported for inactivation of other Atg4 homologs , suggesting that these homologs have tissue-specific functions beyond redundancy .
	manualset3
174762	3	413579	7	NULL	NULL	0	NULL	Atg4 homologs	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings appear to be different than those reported for inactivation of other Atg4 homologs , suggesting that these homologs have tissue-specific functions beyond redundancy .
	manualset3
174763	4	413579	7	NULL	NULL	0	NULL	homologs	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings appear to be different than those reported for inactivation of other Atg4 homologs , suggesting that these homologs have tissue-specific functions beyond redundancy .
	manualset3
174764	5	413579	7	NULL	NULL	0	NULL	tissue-specific functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings appear to be different than those reported for inactivation of other Atg4 homologs , suggesting that these homologs have tissue-specific functions beyond redundancy .
	manualset3
174765	1	413580	7	NULL	NULL	0	NULL	 findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are clinically relevant , as individuals who are colonized with E. histolytica but are resistant to invasive disease have a high prevalence of antibodies to the protective epitope ( s ) , compared to individuals with a history of invasive amebiasis .
	manualset3
174766	2	413580	7	NULL	NULL	0	NULL	 individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are clinically relevant , as individuals who are colonized with E. histolytica but are resistant to invasive disease have a high prevalence of antibodies to the protective epitope ( s ) , compared to individuals with a history of invasive amebiasis .
	manualset3
174767	3	413580	7	NULL	NULL	0	NULL	E. histolytica 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are clinically relevant , as individuals who are colonized with E. histolytica but are resistant to invasive disease have a high prevalence of antibodies to the protective epitope ( s ) , compared to individuals with a history of invasive amebiasis .
	manualset3
174768	4	413580	7	NULL	NULL	0	NULL	invasive disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are clinically relevant , as individuals who are colonized with E. histolytica but are resistant to invasive disease have a high prevalence of antibodies to the protective epitope ( s ) , compared to individuals with a history of invasive amebiasis .
	manualset3
174769	5	413580	7	NULL	NULL	0	NULL	high prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are clinically relevant , as individuals who are colonized with E. histolytica but are resistant to invasive disease have a high prevalence of antibodies to the protective epitope ( s ) , compared to individuals with a history of invasive amebiasis .
	manualset3
174770	6	413580	7	NULL	NULL	0	NULL	antibodies	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are clinically relevant , as individuals who are colonized with E. histolytica but are resistant to invasive disease have a high prevalence of antibodies to the protective epitope ( s ) , compared to individuals with a history of invasive amebiasis .
	manualset3
174771	7	413580	7	NULL	NULL	NULL	NULL	 protective epitope	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings are clinically relevant , as individuals who are colonized with E. histolytica but are resistant to invasive disease have a high prevalence of antibodies to the protective epitope ( s ) , compared to individuals with a history of invasive amebiasis .
	manualset3
174772	8	413580	7	NULL	NULL	0	NULL	individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are clinically relevant , as individuals who are colonized with E. histolytica but are resistant to invasive disease have a high prevalence of antibodies to the protective epitope ( s ) , compared to individuals with a history of invasive amebiasis .
	manualset3
174773	9	413580	7	NULL	NULL	0	NULL	history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are clinically relevant , as individuals who are colonized with E. histolytica but are resistant to invasive disease have a high prevalence of antibodies to the protective epitope ( s ) , compared to individuals with a history of invasive amebiasis .
	manualset3
174774	10	413580	7	NULL	NULL	0	NULL	 invasive amebiasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are clinically relevant , as individuals who are colonized with E. histolytica but are resistant to invasive disease have a high prevalence of antibodies to the protective epitope ( s ) , compared to individuals with a history of invasive amebiasis .
	manualset3
174775	1	413581	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are consistent with HLA class I alleles mediating effective immune control of HIV through the number of p24 Gag-specific CD8 ( + ) T-cell responses generated that can drive significant selection pressure on the virus .
	manualset3
174776	2	413581	7	NULL	NULL	0	NULL	HLA class I alleles	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are consistent with HLA class I alleles mediating effective immune control of HIV through the number of p24 Gag-specific CD8 ( + ) T-cell responses generated that can drive significant selection pressure on the virus .
	manualset3
174777	3	413581	7	NULL	NULL	0	NULL	immune control 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are consistent with HLA class I alleles mediating effective immune control of HIV through the number of p24 Gag-specific CD8 ( + ) T-cell responses generated that can drive significant selection pressure on the virus .
	manualset3
174778	4	413581	7	NULL	NULL	0	NULL	HIV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are consistent with HLA class I alleles mediating effective immune control of HIV through the number of p24 Gag-specific CD8 ( + ) T-cell responses generated that can drive significant selection pressure on the virus .
	manualset3
174779	5	413581	7	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are consistent with HLA class I alleles mediating effective immune control of HIV through the number of p24 Gag-specific CD8 ( + ) T-cell responses generated that can drive significant selection pressure on the virus .
	manualset3
174780	6	413581	7	NULL	NULL	0	NULL	p24 Gag-specific CD8 ( + ) T-cell responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are consistent with HLA class I alleles mediating effective immune control of HIV through the number of p24 Gag-specific CD8 ( + ) T-cell responses generated that can drive significant selection pressure on the virus .
	manualset3
174781	7	413581	7	NULL	NULL	0	NULL	selection pressure	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are consistent with HLA class I alleles mediating effective immune control of HIV through the number of p24 Gag-specific CD8 ( + ) T-cell responses generated that can drive significant selection pressure on the virus .
	manualset3
174782	8	413581	7	NULL	NULL	0	NULL	virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are consistent with HLA class I alleles mediating effective immune control of HIV through the number of p24 Gag-specific CD8 ( + ) T-cell responses generated that can drive significant selection pressure on the virus .
	manualset3
174783	1	413582	7	NULL	NULL	0	NULL	 findings 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are consistent with previous functional and observational studies showing that Asp299 allele , in comparison with Gly299 , is associated with increased TLR4 activation , higher levels of inflammatory cytokines , acute-phase reactants and soluble adhesion molecules , and higher risk of atherosclerosis .
	manualset3
174784	2	413582	7	NULL	NULL	0	NULL	functional studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are consistent with previous functional and observational studies showing that Asp299 allele , in comparison with Gly299 , is associated with increased TLR4 activation , higher levels of inflammatory cytokines , acute-phase reactants and soluble adhesion molecules , and higher risk of atherosclerosis .
	manualset3
174785	3	413582	7	NULL	NULL	0	NULL	 observational studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are consistent with previous functional and observational studies showing that Asp299 allele , in comparison with Gly299 , is associated with increased TLR4 activation , higher levels of inflammatory cytokines , acute-phase reactants and soluble adhesion molecules , and higher risk of atherosclerosis .
	manualset3
174786	4	413582	7	NULL	NULL	0	NULL	Asp299 allele	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are consistent with previous functional and observational studies showing that Asp299 allele , in comparison with Gly299 , is associated with increased TLR4 activation , higher levels of inflammatory cytokines , acute-phase reactants and soluble adhesion molecules , and higher risk of atherosclerosis .
	manualset3
174787	5	413582	7	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are consistent with previous functional and observational studies showing that Asp299 allele , in comparison with Gly299 , is associated with increased TLR4 activation , higher levels of inflammatory cytokines , acute-phase reactants and soluble adhesion molecules , and higher risk of atherosclerosis .
	manualset3
174788	6	413582	7	NULL	NULL	0	NULL	Gly299	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are consistent with previous functional and observational studies showing that Asp299 allele , in comparison with Gly299 , is associated with increased TLR4 activation , higher levels of inflammatory cytokines , acute-phase reactants and soluble adhesion molecules , and higher risk of atherosclerosis .
	manualset3
174789	7	413582	7	NULL	NULL	0	NULL	increased TLR4 activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are consistent with previous functional and observational studies showing that Asp299 allele , in comparison with Gly299 , is associated with increased TLR4 activation , higher levels of inflammatory cytokines , acute-phase reactants and soluble adhesion molecules , and higher risk of atherosclerosis .
	manualset3
174790	8	413582	7	NULL	NULL	0	NULL	higher levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are consistent with previous functional and observational studies showing that Asp299 allele , in comparison with Gly299 , is associated with increased TLR4 activation , higher levels of inflammatory cytokines , acute-phase reactants and soluble adhesion molecules , and higher risk of atherosclerosis .
	manualset3
174791	9	413582	7	NULL	NULL	0	NULL	inflammatory cytokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are consistent with previous functional and observational studies showing that Asp299 allele , in comparison with Gly299 , is associated with increased TLR4 activation , higher levels of inflammatory cytokines , acute-phase reactants and soluble adhesion molecules , and higher risk of atherosclerosis .
	manualset3
174792	10	413582	7	NULL	NULL	0	NULL	acute-phase reactants	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are consistent with previous functional and observational studies showing that Asp299 allele , in comparison with Gly299 , is associated with increased TLR4 activation , higher levels of inflammatory cytokines , acute-phase reactants and soluble adhesion molecules , and higher risk of atherosclerosis .
	manualset3
174793	11	413582	7	NULL	NULL	0	NULL	soluble adhesion molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are consistent with previous functional and observational studies showing that Asp299 allele , in comparison with Gly299 , is associated with increased TLR4 activation , higher levels of inflammatory cytokines , acute-phase reactants and soluble adhesion molecules , and higher risk of atherosclerosis .
	manualset3
174794	12	413582	7	NULL	NULL	0	NULL	higher risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are consistent with previous functional and observational studies showing that Asp299 allele , in comparison with Gly299 , is associated with increased TLR4 activation , higher levels of inflammatory cytokines , acute-phase reactants and soluble adhesion molecules , and higher risk of atherosclerosis .
	manualset3
174795	13	413582	7	NULL	NULL	0	NULL	 atherosclerosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are consistent with previous functional and observational studies showing that Asp299 allele , in comparison with Gly299 , is associated with increased TLR4 activation , higher levels of inflammatory cytokines , acute-phase reactants and soluble adhesion molecules , and higher risk of atherosclerosis .
	manualset3
174796	1	413583	7	NULL	NULL	0	NULL	Adaptation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation of bluetongue virus ( BTV ) to grow in mosquito cells ( C6/36 ) resulted in overexpression of two non-structural proteins ( NS3 and NS3a ) in infected cells .
	manualset3
174797	2	413583	7	NULL	NULL	0	NULL	bluetongue virus ( BTV )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation of bluetongue virus ( BTV ) to grow in mosquito cells ( C6/36 ) resulted in overexpression of two non-structural proteins ( NS3 and NS3a ) in infected cells .
	manualset3
174798	3	413583	7	NULL	NULL	0	NULL	mosquito cells ( C6/36 )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation of bluetongue virus ( BTV ) to grow in mosquito cells ( C6/36 ) resulted in overexpression of two non-structural proteins ( NS3 and NS3a ) in infected cells .
	manualset3
174799	4	413583	7	NULL	NULL	0	NULL	overexpression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation of bluetongue virus ( BTV ) to grow in mosquito cells ( C6/36 ) resulted in overexpression of two non-structural proteins ( NS3 and NS3a ) in infected cells .
	manualset3
174800	5	413583	7	NULL	NULL	0	NULL	two non-structural proteins 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation of bluetongue virus ( BTV ) to grow in mosquito cells ( C6/36 ) resulted in overexpression of two non-structural proteins ( NS3 and NS3a ) in infected cells .
	manualset3
174801	6	413583	7	NULL	NULL	0	NULL	NS3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation of bluetongue virus ( BTV ) to grow in mosquito cells ( C6/36 ) resulted in overexpression of two non-structural proteins ( NS3 and NS3a ) in infected cells .
	manualset3
174802	7	413583	7	NULL	NULL	0	NULL	NS3a	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation of bluetongue virus ( BTV ) to grow in mosquito cells ( C6/36 ) resulted in overexpression of two non-structural proteins ( NS3 and NS3a ) in infected cells .
	manualset3
174803	8	413583	7	NULL	NULL	0	NULL	infected cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation of bluetongue virus ( BTV ) to grow in mosquito cells ( C6/36 ) resulted in overexpression of two non-structural proteins ( NS3 and NS3a ) in infected cells .
	manualset3
174804	1	413584	7	NULL	NULL	0	NULL	 findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are consistent with the idea that the expression of one or more HTLV-I genes may be involved in initiation of transformation , but consistent expression is not needed for maintaining the neoplastic state .
	manualset3
174805	2	413584	7	NULL	NULL	0	NULL	idea	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are consistent with the idea that the expression of one or more HTLV-I genes may be involved in initiation of transformation , but consistent expression is not needed for maintaining the neoplastic state .
	manualset3
174806	3	413584	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are consistent with the idea that the expression of one or more HTLV-I genes may be involved in initiation of transformation , but consistent expression is not needed for maintaining the neoplastic state .
	manualset3
174807	4	413584	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are consistent with the idea that the expression of one or more HTLV-I genes may be involved in initiation of transformation , but consistent expression is not needed for maintaining the neoplastic state .
	manualset3
174808	5	413584	7	NULL	NULL	0	NULL	HTLV-I genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are consistent with the idea that the expression of one or more HTLV-I genes may be involved in initiation of transformation , but consistent expression is not needed for maintaining the neoplastic state .
	manualset3
174809	6	413584	7	NULL	NULL	0	NULL	initiation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are consistent with the idea that the expression of one or more HTLV-I genes may be involved in initiation of transformation , but consistent expression is not needed for maintaining the neoplastic state .
	manualset3
174810	7	413584	7	NULL	NULL	0	NULL	 transformation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are consistent with the idea that the expression of one or more HTLV-I genes may be involved in initiation of transformation , but consistent expression is not needed for maintaining the neoplastic state .
	manualset3
174811	8	413584	7	NULL	NULL	0	NULL	consistent expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are consistent with the idea that the expression of one or more HTLV-I genes may be involved in initiation of transformation , but consistent expression is not needed for maintaining the neoplastic state .
	manualset3
174812	9	413584	7	NULL	NULL	0	NULL	neoplastic state	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are consistent with the idea that the expression of one or more HTLV-I genes may be involved in initiation of transformation , but consistent expression is not needed for maintaining the neoplastic state .
	manualset3
174813	1	413585	7	NULL	NULL	0	NULL	 findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are discussed in terms of severity of illness , level of functioning , and relationships between Axis I and II disorders .
	manualset3
174814	2	413585	7	NULL	NULL	0	NULL	terms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are discussed in terms of severity of illness , level of functioning , and relationships between Axis I and II disorders .
	manualset3
174815	3	413585	7	NULL	NULL	NULL	NULL	severity of illness	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings are discussed in terms of severity of illness , level of functioning , and relationships between Axis I and II disorders .
	manualset3
174816	4	413585	7	NULL	NULL	0	NULL	level of functioning	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are discussed in terms of severity of illness , level of functioning , and relationships between Axis I and II disorders .
	manualset3
174817	5	413585	7	NULL	NULL	0	NULL	relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are discussed in terms of severity of illness , level of functioning , and relationships between Axis I and II disorders .
	manualset3
174818	6	413585	7	NULL	NULL	0	NULL	Axis I disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are discussed in terms of severity of illness , level of functioning , and relationships between Axis I and II disorders .
	manualset3
174819	7	413585	7	NULL	NULL	0	NULL	 Axis II disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings are discussed in terms of severity of illness , level of functioning , and relationships between Axis I and II disorders .
	manualset3
174820	1	413586	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings bear on theories of metacontrast masking by showing that the mechanism giving rise to nonmonotonic masking effects can operate beyond the level of first-order stimulus processing .
	manualset3
174821	2	413586	7	NULL	NULL	NULL	NULL	theories 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings bear on theories of metacontrast masking by showing that the mechanism giving rise to nonmonotonic masking effects can operate beyond the level of first-order stimulus processing .
	manualset3
174823	4	413586	7	NULL	NULL	0	NULL	mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings bear on theories of metacontrast masking by showing that the mechanism giving rise to nonmonotonic masking effects can operate beyond the level of first-order stimulus processing .
	manualset3
174825	5	413586	7	NULL	NULL	NULL	NULL	nonmonotonic masking effects	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings bear on theories of metacontrast masking by showing that the mechanism giving rise to nonmonotonic masking effects can operate beyond the level of first-order stimulus processing .
	manualset3
174826	6	413586	7	NULL	NULL	NULL	NULL	level	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings bear on theories of metacontrast masking by showing that the mechanism giving rise to nonmonotonic masking effects can operate beyond the level of first-order stimulus processing .
	manualset3
174827	7	413586	7	NULL	NULL	NULL	NULL	first-order stimulus processing	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings bear on theories of metacontrast masking by showing that the mechanism giving rise to nonmonotonic masking effects can operate beyond the level of first-order stimulus processing .
	manualset3
177192	8	413586	7	NULL	NULL	0	NULL	metacontrast masking	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings bear on theories of metacontrast masking by showing that the mechanism giving rise to nonmonotonic masking effects can operate beyond the level of first-order stimulus processing .
	manualset3
174828	1	413587	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings challenge the linear rejection-identification model and suggest displaced people may minimize ingroup-outgroup differences , depending on their willingness to seek intergroup contact .
	manualset3
174829	2	413587	7	NULL	NULL	0	NULL	linear rejection-identification model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings challenge the linear rejection-identification model and suggest displaced people may minimize ingroup-outgroup differences , depending on their willingness to seek intergroup contact .
	manualset3
174830	3	413587	7	NULL	NULL	0	NULL	people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings challenge the linear rejection-identification model and suggest displaced people may minimize ingroup-outgroup differences , depending on their willingness to seek intergroup contact .
	manualset3
174831	4	413587	7	NULL	NULL	0	NULL	ingroup-outgroup differences 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings challenge the linear rejection-identification model and suggest displaced people may minimize ingroup-outgroup differences , depending on their willingness to seek intergroup contact .
	manualset3
174832	5	413587	7	NULL	NULL	0	NULL	willingness	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings challenge the linear rejection-identification model and suggest displaced people may minimize ingroup-outgroup differences , depending on their willingness to seek intergroup contact .
	manualset3
174833	6	413587	7	NULL	NULL	0	NULL	 intergroup contact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings challenge the linear rejection-identification model and suggest displaced people may minimize ingroup-outgroup differences , depending on their willingness to seek intergroup contact .
	manualset3
174834	1	413588	7	NULL	NULL	0	NULL	findings 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings contrast with the report that in children under similar conditions only about 50 % of the conversion of fructose to glucose is with cleavage .
	manualset3
174835	2	413588	7	NULL	NULL	0	NULL	report	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings contrast with the report that in children under similar conditions only about 50 % of the conversion of fructose to glucose is with cleavage .
	manualset3
174836	3	413588	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings contrast with the report that in children under similar conditions only about 50 % of the conversion of fructose to glucose is with cleavage .
	manualset3
174837	4	413588	7	NULL	NULL	NULL	NULL	conditions	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings contrast with the report that in children under similar conditions only about 50 % of the conversion of fructose to glucose is with cleavage .
	manualset3
174838	5	413588	7	NULL	NULL	0	NULL	50 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings contrast with the report that in children under similar conditions only about 50 % of the conversion of fructose to glucose is with cleavage .
	manualset3
174839	6	413588	7	NULL	NULL	0	NULL	conversion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings contrast with the report that in children under similar conditions only about 50 % of the conversion of fructose to glucose is with cleavage .
	manualset3
174840	7	413588	7	NULL	NULL	0	NULL	 fructose	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings contrast with the report that in children under similar conditions only about 50 % of the conversion of fructose to glucose is with cleavage .
	manualset3
174841	8	413588	7	NULL	NULL	0	NULL	glucose	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings contrast with the report that in children under similar conditions only about 50 % of the conversion of fructose to glucose is with cleavage .
	manualset3
174842	9	413588	7	NULL	NULL	0	NULL	cleavage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings contrast with the report that in children under similar conditions only about 50 % of the conversion of fructose to glucose is with cleavage .
	manualset3
174843	1	413589	7	NULL	NULL	0	NULL	 findings 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings contrast with those from previous studies and suggest that injections of both S129 phosphorylation mutants result in dopaminergic neurotoxicity similar to wt injections .
	manualset3
174844	2	413589	7	NULL	NULL	0	NULL	previous studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings contrast with those from previous studies and suggest that injections of both S129 phosphorylation mutants result in dopaminergic neurotoxicity similar to wt injections .
	manualset3
174845	3	413589	7	NULL	NULL	0	NULL	injections	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings contrast with those from previous studies and suggest that injections of both S129 phosphorylation mutants result in dopaminergic neurotoxicity similar to wt injections .
	manualset3
174846	4	413589	7	NULL	NULL	0	NULL	S129 phosphorylation mutants	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings contrast with those from previous studies and suggest that injections of both S129 phosphorylation mutants result in dopaminergic neurotoxicity similar to wt injections .
	manualset3
174847	5	413589	7	NULL	NULL	0	NULL	dopaminergic neurotoxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings contrast with those from previous studies and suggest that injections of both S129 phosphorylation mutants result in dopaminergic neurotoxicity similar to wt injections .
	manualset3
174848	6	413589	7	NULL	NULL	0	NULL	wt injections 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings contrast with those from previous studies and suggest that injections of both S129 phosphorylation mutants result in dopaminergic neurotoxicity similar to wt injections .
	manualset3
174849	1	413590	7	NULL	NULL	0	NULL	findings 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings could provide insight into the problem of subendocardial vulnerability to free radical-mediated processes , such as occurs in ischaemia-reperfusion injury .
	manualset3
174850	2	413590	7	NULL	NULL	0	NULL	 insight 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings could provide insight into the problem of subendocardial vulnerability to free radical-mediated processes , such as occurs in ischaemia-reperfusion injury .
	manualset3
174852	3	413590	7	NULL	NULL	0	NULL	problem	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings could provide insight into the problem of subendocardial vulnerability to free radical-mediated processes , such as occurs in ischaemia-reperfusion injury .
	manualset3
174855	4	413590	7	NULL	NULL	0	NULL	subendocardial vulnerability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings could provide insight into the problem of subendocardial vulnerability to free radical-mediated processes , such as occurs in ischaemia-reperfusion injury .
	manualset3
174857	5	413590	7	NULL	NULL	0	NULL	free radical-mediated processes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings could provide insight into the problem of subendocardial vulnerability to free radical-mediated processes , such as occurs in ischaemia-reperfusion injury .
	manualset3
174858	6	413590	7	NULL	NULL	0	NULL	ischaemia-reperfusion injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings could provide insight into the problem of subendocardial vulnerability to free radical-mediated processes , such as occurs in ischaemia-reperfusion injury .
	manualset3
174863	1	413591	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings demonstrate that higher levels of activity are associated with better physical health in elderly persons , as indicated by less frequent and shorter hospital stays , and lower frequency of surgical interventions .
	manualset3
174865	2	413591	7	NULL	NULL	0	NULL	higher levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings demonstrate that higher levels of activity are associated with better physical health in elderly persons , as indicated by less frequent and shorter hospital stays , and lower frequency of surgical interventions .
	manualset3
174868	3	413591	7	NULL	NULL	0	NULL	activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings demonstrate that higher levels of activity are associated with better physical health in elderly persons , as indicated by less frequent and shorter hospital stays , and lower frequency of surgical interventions .
	manualset3
174871	4	413591	7	NULL	NULL	0	NULL	physical health	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings demonstrate that higher levels of activity are associated with better physical health in elderly persons , as indicated by less frequent and shorter hospital stays , and lower frequency of surgical interventions .
	manualset3
174873	5	413591	7	NULL	NULL	0	NULL	elderly persons	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings demonstrate that higher levels of activity are associated with better physical health in elderly persons , as indicated by less frequent and shorter hospital stays , and lower frequency of surgical interventions .
	manualset3
174877	6	413591	7	NULL	NULL	0	NULL	shorter hospital stays	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings demonstrate that higher levels of activity are associated with better physical health in elderly persons , as indicated by less frequent and shorter hospital stays , and lower frequency of surgical interventions .
	manualset3
174879	7	413591	7	NULL	NULL	0	NULL	lower frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings demonstrate that higher levels of activity are associated with better physical health in elderly persons , as indicated by less frequent and shorter hospital stays , and lower frequency of surgical interventions .
	manualset3
174880	8	413591	7	NULL	NULL	0	NULL	surgical interventions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings demonstrate that higher levels of activity are associated with better physical health in elderly persons , as indicated by less frequent and shorter hospital stays , and lower frequency of surgical interventions .
	manualset3
174892	1	413592	7	NULL	NULL	NULL	NULL	Adaptation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Adaptation to high altitude hypoxia was created by placing the animals daily for 5 hours , into an altitude chamber , at an `` altitude '' of 6000 m. The degree of hypertrophy of the right ventricle and its RNA content was studied after 20 days of adaptation , as well as 2 , 10 , 20 and 40 days after cessation of hypoxia .
	manualset3
174904	2	413592	7	NULL	NULL	0	NULL	high altitude hypoxia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation to high altitude hypoxia was created by placing the animals daily for 5 hours , into an altitude chamber , at an `` altitude '' of 6000 m. The degree of hypertrophy of the right ventricle and its RNA content was studied after 20 days of adaptation , as well as 2 , 10 , 20 and 40 days after cessation of hypoxia .
	manualset3
174907	3	413592	7	NULL	NULL	0	NULL	animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation to high altitude hypoxia was created by placing the animals daily for 5 hours , into an altitude chamber , at an `` altitude '' of 6000 m. The degree of hypertrophy of the right ventricle and its RNA content was studied after 20 days of adaptation , as well as 2 , 10 , 20 and 40 days after cessation of hypoxia .
	manualset3
174909	4	413592	7	NULL	NULL	0	NULL	5 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation to high altitude hypoxia was created by placing the animals daily for 5 hours , into an altitude chamber , at an `` altitude '' of 6000 m. The degree of hypertrophy of the right ventricle and its RNA content was studied after 20 days of adaptation , as well as 2 , 10 , 20 and 40 days after cessation of hypoxia .
	manualset3
174916	5	413592	7	NULL	NULL	0	NULL	altitude chamber	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation to high altitude hypoxia was created by placing the animals daily for 5 hours , into an altitude chamber , at an `` altitude '' of 6000 m. The degree of hypertrophy of the right ventricle and its RNA content was studied after 20 days of adaptation , as well as 2 , 10 , 20 and 40 days after cessation of hypoxia .
	manualset3
174918	6	413592	7	NULL	NULL	0	NULL	altitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation to high altitude hypoxia was created by placing the animals daily for 5 hours , into an altitude chamber , at an `` altitude '' of 6000 m. The degree of hypertrophy of the right ventricle and its RNA content was studied after 20 days of adaptation , as well as 2 , 10 , 20 and 40 days after cessation of hypoxia .
	manualset3
174921	7	413592	7	NULL	NULL	0	NULL	 6000 m	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation to high altitude hypoxia was created by placing the animals daily for 5 hours , into an altitude chamber , at an `` altitude '' of 6000 m. The degree of hypertrophy of the right ventricle and its RNA content was studied after 20 days of adaptation , as well as 2 , 10 , 20 and 40 days after cessation of hypoxia .
	manualset3
174922	8	413592	7	NULL	NULL	0	NULL	degree	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation to high altitude hypoxia was created by placing the animals daily for 5 hours , into an altitude chamber , at an `` altitude '' of 6000 m. The degree of hypertrophy of the right ventricle and its RNA content was studied after 20 days of adaptation , as well as 2 , 10 , 20 and 40 days after cessation of hypoxia .
	manualset3
174923	9	413592	7	NULL	NULL	0	NULL	hypertrophy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation to high altitude hypoxia was created by placing the animals daily for 5 hours , into an altitude chamber , at an `` altitude '' of 6000 m. The degree of hypertrophy of the right ventricle and its RNA content was studied after 20 days of adaptation , as well as 2 , 10 , 20 and 40 days after cessation of hypoxia .
	manualset3
174924	10	413592	7	NULL	NULL	0	NULL	right ventricle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation to high altitude hypoxia was created by placing the animals daily for 5 hours , into an altitude chamber , at an `` altitude '' of 6000 m. The degree of hypertrophy of the right ventricle and its RNA content was studied after 20 days of adaptation , as well as 2 , 10 , 20 and 40 days after cessation of hypoxia .
	manualset3
174926	11	413592	7	NULL	NULL	NULL	NULL	RNA content 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Adaptation to high altitude hypoxia was created by placing the animals daily for 5 hours , into an altitude chamber , at an `` altitude '' of 6000 m. The degree of hypertrophy of the right ventricle and its RNA content was studied after 20 days of adaptation , as well as 2 , 10 , 20 and 40 days after cessation of hypoxia .
	manualset3
174929	12	413592	7	NULL	NULL	0	NULL	20 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation to high altitude hypoxia was created by placing the animals daily for 5 hours , into an altitude chamber , at an `` altitude '' of 6000 m. The degree of hypertrophy of the right ventricle and its RNA content was studied after 20 days of adaptation , as well as 2 , 10 , 20 and 40 days after cessation of hypoxia .
	manualset3
174930	13	413592	7	NULL	NULL	NULL	NULL	adaptation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Adaptation to high altitude hypoxia was created by placing the animals daily for 5 hours , into an altitude chamber , at an `` altitude '' of 6000 m. The degree of hypertrophy of the right ventricle and its RNA content was studied after 20 days of adaptation , as well as 2 , 10 , 20 and 40 days after cessation of hypoxia .
	manualset3
174931	14	413592	7	NULL	NULL	0	NULL	2 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation to high altitude hypoxia was created by placing the animals daily for 5 hours , into an altitude chamber , at an `` altitude '' of 6000 m. The degree of hypertrophy of the right ventricle and its RNA content was studied after 20 days of adaptation , as well as 2 , 10 , 20 and 40 days after cessation of hypoxia .
	manualset3
174934	15	413592	7	NULL	NULL	0	NULL	10 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation to high altitude hypoxia was created by placing the animals daily for 5 hours , into an altitude chamber , at an `` altitude '' of 6000 m. The degree of hypertrophy of the right ventricle and its RNA content was studied after 20 days of adaptation , as well as 2 , 10 , 20 and 40 days after cessation of hypoxia .
	manualset3
174936	16	413592	7	NULL	NULL	0	NULL	20 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation to high altitude hypoxia was created by placing the animals daily for 5 hours , into an altitude chamber , at an `` altitude '' of 6000 m. The degree of hypertrophy of the right ventricle and its RNA content was studied after 20 days of adaptation , as well as 2 , 10 , 20 and 40 days after cessation of hypoxia .
	manualset3
174940	17	413592	7	NULL	NULL	NULL	NULL	40 days	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Adaptation to high altitude hypoxia was created by placing the animals daily for 5 hours , into an altitude chamber , at an `` altitude '' of 6000 m. The degree of hypertrophy of the right ventricle and its RNA content was studied after 20 days of adaptation , as well as 2 , 10 , 20 and 40 days after cessation of hypoxia .
	manualset3
174942	18	413592	7	NULL	NULL	NULL	NULL	cessation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Adaptation to high altitude hypoxia was created by placing the animals daily for 5 hours , into an altitude chamber , at an `` altitude '' of 6000 m. The degree of hypertrophy of the right ventricle and its RNA content was studied after 20 days of adaptation , as well as 2 , 10 , 20 and 40 days after cessation of hypoxia .
	manualset3
174943	19	413592	7	NULL	NULL	0	NULL	hypoxia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation to high altitude hypoxia was created by placing the animals daily for 5 hours , into an altitude chamber , at an `` altitude '' of 6000 m. The degree of hypertrophy of the right ventricle and its RNA content was studied after 20 days of adaptation , as well as 2 , 10 , 20 and 40 days after cessation of hypoxia .
	manualset3
178885	20	413592	7	NULL	NULL	0	NULL	placing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation to high altitude hypoxia was created by placing the animals daily for 5 hours , into an altitude chamber , at an `` altitude '' of 6000 m. The degree of hypertrophy of the right ventricle and its RNA content was studied after 20 days of adaptation , as well as 2 , 10 , 20 and 40 days after cessation of hypoxia .
	manualset3
174950	1	413593	7	NULL	NULL	0	NULL	 findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings demonstrate that in hemodialysis patients PCR is necessary for the diagnosis of HCV infection .
	manualset3
174952	2	413593	7	NULL	NULL	0	NULL	hemodialysis patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings demonstrate that in hemodialysis patients PCR is necessary for the diagnosis of HCV infection .
	manualset3
174953	3	413593	7	NULL	NULL	0	NULL	PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings demonstrate that in hemodialysis patients PCR is necessary for the diagnosis of HCV infection .
	manualset3
174954	4	413593	7	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings demonstrate that in hemodialysis patients PCR is necessary for the diagnosis of HCV infection .
	manualset3
174955	5	413593	7	NULL	NULL	0	NULL	HCV infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings demonstrate that in hemodialysis patients PCR is necessary for the diagnosis of HCV infection .
	manualset3
174975	1	413594	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings demonstrate that maintaining endothelial barrier function is dependent upon active R-Ras and association between R-Ras and FLNa and that loss of this interaction promotes VE-Cadherin phosphorylation and changes in downstream effectors that lead to endothelial leakiness .
	manualset3
174976	2	413594	7	NULL	NULL	0	NULL	endothelial barrier function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings demonstrate that maintaining endothelial barrier function is dependent upon active R-Ras and association between R-Ras and FLNa and that loss of this interaction promotes VE-Cadherin phosphorylation and changes in downstream effectors that lead to endothelial leakiness .
	manualset3
174977	3	413594	7	NULL	NULL	0	NULL	active R-Ras 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings demonstrate that maintaining endothelial barrier function is dependent upon active R-Ras and association between R-Ras and FLNa and that loss of this interaction promotes VE-Cadherin phosphorylation and changes in downstream effectors that lead to endothelial leakiness .
	manualset3
174978	4	413594	7	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings demonstrate that maintaining endothelial barrier function is dependent upon active R-Ras and association between R-Ras and FLNa and that loss of this interaction promotes VE-Cadherin phosphorylation and changes in downstream effectors that lead to endothelial leakiness .
	manualset3
174979	5	413594	7	NULL	NULL	NULL	NULL	R-Ras	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings demonstrate that maintaining endothelial barrier function is dependent upon active R-Ras and association between R-Ras and FLNa and that loss of this interaction promotes VE-Cadherin phosphorylation and changes in downstream effectors that lead to endothelial leakiness .
	manualset3
174980	6	413594	7	NULL	NULL	NULL	NULL	FLNa	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings demonstrate that maintaining endothelial barrier function is dependent upon active R-Ras and association between R-Ras and FLNa and that loss of this interaction promotes VE-Cadherin phosphorylation and changes in downstream effectors that lead to endothelial leakiness .
	manualset3
174981	7	413594	7	NULL	NULL	0	NULL	loss	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings demonstrate that maintaining endothelial barrier function is dependent upon active R-Ras and association between R-Ras and FLNa and that loss of this interaction promotes VE-Cadherin phosphorylation and changes in downstream effectors that lead to endothelial leakiness .
	manualset3
174982	8	413594	7	NULL	NULL	0	NULL	interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings demonstrate that maintaining endothelial barrier function is dependent upon active R-Ras and association between R-Ras and FLNa and that loss of this interaction promotes VE-Cadherin phosphorylation and changes in downstream effectors that lead to endothelial leakiness .
	manualset3
174983	9	413594	7	NULL	NULL	0	NULL	VE-Cadherin phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings demonstrate that maintaining endothelial barrier function is dependent upon active R-Ras and association between R-Ras and FLNa and that loss of this interaction promotes VE-Cadherin phosphorylation and changes in downstream effectors that lead to endothelial leakiness .
	manualset3
174984	10	413594	7	NULL	NULL	0	NULL	changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings demonstrate that maintaining endothelial barrier function is dependent upon active R-Ras and association between R-Ras and FLNa and that loss of this interaction promotes VE-Cadherin phosphorylation and changes in downstream effectors that lead to endothelial leakiness .
	manualset3
174985	11	413594	7	NULL	NULL	0	NULL	downstream effectors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings demonstrate that maintaining endothelial barrier function is dependent upon active R-Ras and association between R-Ras and FLNa and that loss of this interaction promotes VE-Cadherin phosphorylation and changes in downstream effectors that lead to endothelial leakiness .
	manualset3
174986	12	413594	7	NULL	NULL	0	NULL	endothelial leakiness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings demonstrate that maintaining endothelial barrier function is dependent upon active R-Ras and association between R-Ras and FLNa and that loss of this interaction promotes VE-Cadherin phosphorylation and changes in downstream effectors that lead to endothelial leakiness .
	manualset3
174987	1	413595	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings emphasize the potential of the tetraamine backbone as a pharmacophore to modulate NMDA receptor-channel function .
	manualset3
174988	2	413595	7	NULL	NULL	NULL	NULL	 potential	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings emphasize the potential of the tetraamine backbone as a pharmacophore to modulate NMDA receptor-channel function .
	manualset3
174989	3	413595	7	NULL	NULL	0	NULL	 tetraamine backbone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings emphasize the potential of the tetraamine backbone as a pharmacophore to modulate NMDA receptor-channel function .
	manualset3
174990	4	413595	7	NULL	NULL	0	NULL	pharmacophore 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings emphasize the potential of the tetraamine backbone as a pharmacophore to modulate NMDA receptor-channel function .
	manualset3
174991	5	413595	7	NULL	NULL	0	NULL	NMDA receptor-channel function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings emphasize the potential of the tetraamine backbone as a pharmacophore to modulate NMDA receptor-channel function .
	manualset3
174992	1	413596	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings greatly facilitate the purification of AcAPc2 and are very important for the additional studies on its anti-coagulation mechanism and its clinical application as anti-coagulation medicine .
	manualset3
174993	2	413596	7	NULL	NULL	0	NULL	purification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings greatly facilitate the purification of AcAPc2 and are very important for the additional studies on its anti-coagulation mechanism and its clinical application as anti-coagulation medicine .
	manualset3
174994	3	413596	7	NULL	NULL	0	NULL	AcAPc2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings greatly facilitate the purification of AcAPc2 and are very important for the additional studies on its anti-coagulation mechanism and its clinical application as anti-coagulation medicine .
	manualset3
174995	4	413596	7	NULL	NULL	0	NULL	important	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings greatly facilitate the purification of AcAPc2 and are very important for the additional studies on its anti-coagulation mechanism and its clinical application as anti-coagulation medicine .
	manualset3
174996	5	413596	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings greatly facilitate the purification of AcAPc2 and are very important for the additional studies on its anti-coagulation mechanism and its clinical application as anti-coagulation medicine .
	manualset3
174997	6	413596	7	NULL	NULL	0	NULL	anti-coagulation mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings greatly facilitate the purification of AcAPc2 and are very important for the additional studies on its anti-coagulation mechanism and its clinical application as anti-coagulation medicine .
	manualset3
174998	7	413596	7	NULL	NULL	0	NULL	clinical application	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings greatly facilitate the purification of AcAPc2 and are very important for the additional studies on its anti-coagulation mechanism and its clinical application as anti-coagulation medicine .
	manualset3
174999	8	413596	7	NULL	NULL	NULL	NULL	anti-coagulation medicine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings greatly facilitate the purification of AcAPc2 and are very important for the additional studies on its anti-coagulation mechanism and its clinical application as anti-coagulation medicine .
	manualset3
175000	1	413597	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings have important implications in the search for effective neuroprotective therapies in treating stroke .
	manualset3
175001	2	413597	7	NULL	NULL	0	NULL	implications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings have important implications in the search for effective neuroprotective therapies in treating stroke .
	manualset3
175002	3	413597	7	NULL	NULL	0	NULL	search	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings have important implications in the search for effective neuroprotective therapies in treating stroke .
	manualset3
175003	4	413597	7	NULL	NULL	0	NULL	effective neuroprotective therapies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings have important implications in the search for effective neuroprotective therapies in treating stroke .
	manualset3
175004	5	413597	7	NULL	NULL	0	NULL	stroke	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings have important implications in the search for effective neuroprotective therapies in treating stroke .
	manualset3
175005	1	413598	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings highlight the importance of white matter integrity in working memory performance associated with normal aging .
	manualset3
175006	2	413598	7	NULL	NULL	0	NULL	white matter integrity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings highlight the importance of white matter integrity in working memory performance associated with normal aging .
	manualset3
175007	3	413598	7	NULL	NULL	NULL	NULL	 working memory performance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings highlight the importance of white matter integrity in working memory performance associated with normal aging .
	manualset3
175008	4	413598	7	NULL	NULL	0	NULL	normal aging	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings highlight the importance of white matter integrity in working memory performance associated with normal aging .
	manualset3
190509	5	413598	7	NULL	NULL	0	NULL	 importance	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings highlight the importance of white matter integrity in working memory performance associated with normal aging .
	manualset3
175009	1	413599	7	NULL	NULL	NULL	NULL	Adaptation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Adaptation to sour arises from the activation of the basolateral sodium-hydrogen exchanger isoform-1 by an increase in intracellular calcium that sustains the tonic phase of the sour taste response .
	manualset3
175010	2	413599	7	NULL	NULL	NULL	NULL	sour	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Adaptation to sour arises from the activation of the basolateral sodium-hydrogen exchanger isoform-1 by an increase in intracellular calcium that sustains the tonic phase of the sour taste response .
	manualset3
175011	3	413599	7	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation to sour arises from the activation of the basolateral sodium-hydrogen exchanger isoform-1 by an increase in intracellular calcium that sustains the tonic phase of the sour taste response .
	manualset3
175012	4	413599	7	NULL	NULL	0	NULL	basolateral sodium-hydrogen exchanger isoform-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation to sour arises from the activation of the basolateral sodium-hydrogen exchanger isoform-1 by an increase in intracellular calcium that sustains the tonic phase of the sour taste response .
	manualset3
175013	5	413599	7	NULL	NULL	0	NULL	increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation to sour arises from the activation of the basolateral sodium-hydrogen exchanger isoform-1 by an increase in intracellular calcium that sustains the tonic phase of the sour taste response .
	manualset3
175014	6	413599	7	NULL	NULL	0	NULL	intracellular calcium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation to sour arises from the activation of the basolateral sodium-hydrogen exchanger isoform-1 by an increase in intracellular calcium that sustains the tonic phase of the sour taste response .
	manualset3
175015	7	413599	7	NULL	NULL	0	NULL	tonic phase	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation to sour arises from the activation of the basolateral sodium-hydrogen exchanger isoform-1 by an increase in intracellular calcium that sustains the tonic phase of the sour taste response .
	manualset3
175016	8	413599	7	NULL	NULL	0	NULL	sour taste response 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation to sour arises from the activation of the basolateral sodium-hydrogen exchanger isoform-1 by an increase in intracellular calcium that sustains the tonic phase of the sour taste response .
	manualset3
175017	1	413600	7	NULL	NULL	0	NULL	 findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings illustrate that self-reactive CD8 T cells can play an important innate function in the early defense against bacterial infection .
	manualset3
175018	2	413600	7	NULL	NULL	0	NULL	self-reactive CD8 T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings illustrate that self-reactive CD8 T cells can play an important innate function in the early defense against bacterial infection .
	manualset3
175019	3	413600	7	NULL	NULL	0	NULL	 innate function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings illustrate that self-reactive CD8 T cells can play an important innate function in the early defense against bacterial infection .
	manualset3
175020	4	413600	7	NULL	NULL	0	NULL	early defense	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings illustrate that self-reactive CD8 T cells can play an important innate function in the early defense against bacterial infection .
	manualset3
175021	5	413600	7	NULL	NULL	0	NULL	bacterial infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings illustrate that self-reactive CD8 T cells can play an important innate function in the early defense against bacterial infection .
	manualset3
175022	1	413601	7	NULL	NULL	0	NULL	findings 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings implicate the snowshoe hare as a possible mammalian amplifying host for WEE virus in the boreal forest .
	manualset3
175023	2	413601	7	NULL	NULL	0	NULL	 snowshoe hare	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings implicate the snowshoe hare as a possible mammalian amplifying host for WEE virus in the boreal forest .
	manualset3
175024	3	413601	7	NULL	NULL	0	NULL	mammalian amplifying host	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings implicate the snowshoe hare as a possible mammalian amplifying host for WEE virus in the boreal forest .
	manualset3
175025	4	413601	7	NULL	NULL	0	NULL	WEE virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings implicate the snowshoe hare as a possible mammalian amplifying host for WEE virus in the boreal forest .
	manualset3
175026	5	413601	7	NULL	NULL	0	NULL	boreal forest	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings implicate the snowshoe hare as a possible mammalian amplifying host for WEE virus in the boreal forest .
	manualset3
175027	1	413602	7	NULL	NULL	0	NULL	 findings 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings imply that an input image can be efficiently represented by ICA bases .
	manualset3
175028	2	413602	7	NULL	NULL	NULL	NULL	input image	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings imply that an input image can be efficiently represented by ICA bases .
	manualset3
175029	3	413602	7	NULL	NULL	0	NULL	 ICA bases 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings imply that an input image can be efficiently represented by ICA bases .
	manualset3
175030	1	413603	7	NULL	NULL	0	NULL	 findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate an inverse relationship between survivin and bcl-2 expression and suggest that these two inhibitors of apoptosis function through different pathways in the regulation of tumorigenesis in NSCLC .
	manualset3
175031	2	413603	7	NULL	NULL	0	NULL	inverse relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate an inverse relationship between survivin and bcl-2 expression and suggest that these two inhibitors of apoptosis function through different pathways in the regulation of tumorigenesis in NSCLC .
	manualset3
175032	3	413603	7	NULL	NULL	0	NULL	survivin	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate an inverse relationship between survivin and bcl-2 expression and suggest that these two inhibitors of apoptosis function through different pathways in the regulation of tumorigenesis in NSCLC .
	manualset3
175033	4	413603	7	NULL	NULL	NULL	NULL	bcl-2 expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings indicate an inverse relationship between survivin and bcl-2 expression and suggest that these two inhibitors of apoptosis function through different pathways in the regulation of tumorigenesis in NSCLC .
	manualset3
175034	5	413603	7	NULL	NULL	0	NULL	 two inhibitors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate an inverse relationship between survivin and bcl-2 expression and suggest that these two inhibitors of apoptosis function through different pathways in the regulation of tumorigenesis in NSCLC .
	manualset3
175035	6	413603	7	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate an inverse relationship between survivin and bcl-2 expression and suggest that these two inhibitors of apoptosis function through different pathways in the regulation of tumorigenesis in NSCLC .
	manualset3
175036	7	413603	7	NULL	NULL	0	NULL	pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate an inverse relationship between survivin and bcl-2 expression and suggest that these two inhibitors of apoptosis function through different pathways in the regulation of tumorigenesis in NSCLC .
	manualset3
175037	8	413603	7	NULL	NULL	0	NULL	 regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate an inverse relationship between survivin and bcl-2 expression and suggest that these two inhibitors of apoptosis function through different pathways in the regulation of tumorigenesis in NSCLC .
	manualset3
175038	9	413603	7	NULL	NULL	0	NULL	tumorigenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate an inverse relationship between survivin and bcl-2 expression and suggest that these two inhibitors of apoptosis function through different pathways in the regulation of tumorigenesis in NSCLC .
	manualset3
175039	10	413603	7	NULL	NULL	0	NULL	NSCLC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate an inverse relationship between survivin and bcl-2 expression and suggest that these two inhibitors of apoptosis function through different pathways in the regulation of tumorigenesis in NSCLC .
	manualset3
175040	1	413604	7	NULL	NULL	0	NULL	 findings 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate prolactin may have a primary dipsogenic activity .
	manualset3
175041	2	413604	7	NULL	NULL	0	NULL	prolactin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate prolactin may have a primary dipsogenic activity .
	manualset3
175042	3	413604	7	NULL	NULL	0	NULL	primary dipsogenic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate prolactin may have a primary dipsogenic activity .
	manualset3
175043	1	413605	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that a mutation hotspot exists in the Ca locus .
	manualset3
175044	2	413605	7	NULL	NULL	0	NULL	mutation hotspot	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that a mutation hotspot exists in the Ca locus .
	manualset3
175045	3	413605	7	NULL	NULL	0	NULL	Ca locus 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that a mutation hotspot exists in the Ca locus .
	manualset3
175046	1	413606	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that caution may be warranted in relying exclusively on SNP databases as catalogs for polymorphic signaling protein genes .
	manualset3
175047	2	413606	7	NULL	NULL	0	NULL	caution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that caution may be warranted in relying exclusively on SNP databases as catalogs for polymorphic signaling protein genes .
	manualset3
175048	3	413606	7	NULL	NULL	NULL	NULL	SNP databases	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings indicate that caution may be warranted in relying exclusively on SNP databases as catalogs for polymorphic signaling protein genes .
	manualset3
175049	4	413606	7	NULL	NULL	0	NULL	 catalogs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that caution may be warranted in relying exclusively on SNP databases as catalogs for polymorphic signaling protein genes .
	manualset3
175050	5	413606	7	NULL	NULL	0	NULL	polymorphic signaling protein genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that caution may be warranted in relying exclusively on SNP databases as catalogs for polymorphic signaling protein genes .
	manualset3
175051	1	413607	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that cell-mediated tumor cell destruction rather than antiviral reaction induces systemic spontaneous regression of multiple papillomas in man .
	manualset3
175052	2	413607	7	NULL	NULL	0	NULL	cell-mediated tumor cell destruction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that cell-mediated tumor cell destruction rather than antiviral reaction induces systemic spontaneous regression of multiple papillomas in man .
	manualset3
175053	3	413607	7	NULL	NULL	0	NULL	antiviral reaction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that cell-mediated tumor cell destruction rather than antiviral reaction induces systemic spontaneous regression of multiple papillomas in man .
	manualset3
175054	4	413607	7	NULL	NULL	0	NULL	systemic spontaneous regression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that cell-mediated tumor cell destruction rather than antiviral reaction induces systemic spontaneous regression of multiple papillomas in man .
	manualset3
175055	5	413607	7	NULL	NULL	NULL	NULL	 multiple papillomas	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings indicate that cell-mediated tumor cell destruction rather than antiviral reaction induces systemic spontaneous regression of multiple papillomas in man .
	manualset3
175056	6	413607	7	NULL	NULL	0	NULL	man 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that cell-mediated tumor cell destruction rather than antiviral reaction induces systemic spontaneous regression of multiple papillomas in man .
	manualset3
175057	1	413608	7	NULL	NULL	0	NULL	 findings 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that classification accuracy statistics , most notably predictive values and risk ratios , are potentially underused in neuropsychology .
	manualset3
175058	2	413608	7	NULL	NULL	0	NULL	classification accuracy statistics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that classification accuracy statistics , most notably predictive values and risk ratios , are potentially underused in neuropsychology .
	manualset3
175059	3	413608	7	NULL	NULL	0	NULL	predictive values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that classification accuracy statistics , most notably predictive values and risk ratios , are potentially underused in neuropsychology .
	manualset3
175060	4	413608	7	NULL	NULL	0	NULL	 risk ratios	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that classification accuracy statistics , most notably predictive values and risk ratios , are potentially underused in neuropsychology .
	manualset3
175061	5	413608	7	NULL	NULL	0	NULL	neuropsychology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that classification accuracy statistics , most notably predictive values and risk ratios , are potentially underused in neuropsychology .
	manualset3
175062	1	413609	7	NULL	NULL	0	NULL	findings 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that increased ADA expression in ATL cells reflects increased transcriptional activity for the ADA gene or increased stability of ADA mRNA .
	manualset3
175063	2	413609	7	NULL	NULL	0	NULL	increased ADA expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that increased ADA expression in ATL cells reflects increased transcriptional activity for the ADA gene or increased stability of ADA mRNA .
	manualset3
175064	3	413609	7	NULL	NULL	0	NULL	ATL cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that increased ADA expression in ATL cells reflects increased transcriptional activity for the ADA gene or increased stability of ADA mRNA .
	manualset3
175065	4	413609	7	NULL	NULL	0	NULL	increased transcriptional activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that increased ADA expression in ATL cells reflects increased transcriptional activity for the ADA gene or increased stability of ADA mRNA .
	manualset3
175066	5	413609	7	NULL	NULL	0	NULL	ADA gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that increased ADA expression in ATL cells reflects increased transcriptional activity for the ADA gene or increased stability of ADA mRNA .
	manualset3
175067	6	413609	7	NULL	NULL	0	NULL	increased stability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that increased ADA expression in ATL cells reflects increased transcriptional activity for the ADA gene or increased stability of ADA mRNA .
	manualset3
175068	7	413609	7	NULL	NULL	0	NULL	ADA mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that increased ADA expression in ATL cells reflects increased transcriptional activity for the ADA gene or increased stability of ADA mRNA .
	manualset3
175069	1	413610	7	NULL	NULL	0	NULL	 findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that microtubules function in the organization of the Golgi complex in osteoblasts .
	manualset3
175070	2	413610	7	NULL	NULL	0	NULL	microtubules	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that microtubules function in the organization of the Golgi complex in osteoblasts .
	manualset3
175071	3	413610	7	NULL	NULL	0	NULL	function 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that microtubules function in the organization of the Golgi complex in osteoblasts .
	manualset3
175072	4	413610	7	NULL	NULL	0	NULL	 organization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that microtubules function in the organization of the Golgi complex in osteoblasts .
	manualset3
175073	5	413610	7	NULL	NULL	0	NULL	Golgi complex	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that microtubules function in the organization of the Golgi complex in osteoblasts .
	manualset3
175074	6	413610	7	NULL	NULL	0	NULL	osteoblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that microtubules function in the organization of the Golgi complex in osteoblasts .
	manualset3
175075	1	413611	7	NULL	NULL	0	NULL	 findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that raf kinase , when activated by a transmembrane signal or by mutation of a regulatory domain , can phosphorylate a factor ( s ) capable of regulating transcription of the c-fos and actin genes .
	manualset3
175076	2	413611	7	NULL	NULL	0	NULL	 raf kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that raf kinase , when activated by a transmembrane signal or by mutation of a regulatory domain , can phosphorylate a factor ( s ) capable of regulating transcription of the c-fos and actin genes .
	manualset3
175077	3	413611	7	NULL	NULL	0	NULL	transmembrane signal	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that raf kinase , when activated by a transmembrane signal or by mutation of a regulatory domain , can phosphorylate a factor ( s ) capable of regulating transcription of the c-fos and actin genes .
	manualset3
175078	4	413611	7	NULL	NULL	0	NULL	mutation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that raf kinase , when activated by a transmembrane signal or by mutation of a regulatory domain , can phosphorylate a factor ( s ) capable of regulating transcription of the c-fos and actin genes .
	manualset3
175079	5	413611	7	NULL	NULL	0	NULL	regulatory domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that raf kinase , when activated by a transmembrane signal or by mutation of a regulatory domain , can phosphorylate a factor ( s ) capable of regulating transcription of the c-fos and actin genes .
	manualset3
175080	6	413611	7	NULL	NULL	0	NULL	factor ( s ) 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that raf kinase , when activated by a transmembrane signal or by mutation of a regulatory domain , can phosphorylate a factor ( s ) capable of regulating transcription of the c-fos and actin genes .
	manualset3
175081	7	413611	7	NULL	NULL	0	NULL	transcription 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that raf kinase , when activated by a transmembrane signal or by mutation of a regulatory domain , can phosphorylate a factor ( s ) capable of regulating transcription of the c-fos and actin genes .
	manualset3
175082	8	413611	7	NULL	NULL	0	NULL	 c-fos genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that raf kinase , when activated by a transmembrane signal or by mutation of a regulatory domain , can phosphorylate a factor ( s ) capable of regulating transcription of the c-fos and actin genes .
	manualset3
175083	9	413611	7	NULL	NULL	0	NULL	actin genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that raf kinase , when activated by a transmembrane signal or by mutation of a regulatory domain , can phosphorylate a factor ( s ) capable of regulating transcription of the c-fos and actin genes .
	manualset3
175084	1	413612	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that reactive oxygen intermediates , the transcription factor Egr-1 , and p44/42 MAPK are critical elements in the transcriptional regulation of the SERCA2 gene in response to DOX .
	manualset3
175085	2	413612	7	NULL	NULL	0	NULL	reactive oxygen intermediates	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that reactive oxygen intermediates , the transcription factor Egr-1 , and p44/42 MAPK are critical elements in the transcriptional regulation of the SERCA2 gene in response to DOX .
	manualset3
175086	3	413612	7	NULL	NULL	NULL	NULL	transcription factor Egr-1	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings indicate that reactive oxygen intermediates , the transcription factor Egr-1 , and p44/42 MAPK are critical elements in the transcriptional regulation of the SERCA2 gene in response to DOX .
	manualset3
175087	4	413612	7	NULL	NULL	NULL	NULL	 p44/42 MAPK	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings indicate that reactive oxygen intermediates , the transcription factor Egr-1 , and p44/42 MAPK are critical elements in the transcriptional regulation of the SERCA2 gene in response to DOX .
	manualset3
175088	5	413612	7	NULL	NULL	0	NULL	elements	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that reactive oxygen intermediates , the transcription factor Egr-1 , and p44/42 MAPK are critical elements in the transcriptional regulation of the SERCA2 gene in response to DOX .
	manualset3
175089	6	413612	7	NULL	NULL	0	NULL	transcriptional regulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that reactive oxygen intermediates , the transcription factor Egr-1 , and p44/42 MAPK are critical elements in the transcriptional regulation of the SERCA2 gene in response to DOX .
	manualset3
175090	7	413612	7	NULL	NULL	0	NULL	 SERCA2 gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that reactive oxygen intermediates , the transcription factor Egr-1 , and p44/42 MAPK are critical elements in the transcriptional regulation of the SERCA2 gene in response to DOX .
	manualset3
175091	8	413612	7	NULL	NULL	0	NULL	 DOX	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that reactive oxygen intermediates , the transcription factor Egr-1 , and p44/42 MAPK are critical elements in the transcriptional regulation of the SERCA2 gene in response to DOX .
	manualset3
175092	1	413613	7	NULL	NULL	0	NULL	 findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that sCT inhibits gastric acid secretion via receptors localized in the hypothalamus and in adjacent areas of the brain .
	manualset3
175093	2	413613	7	NULL	NULL	0	NULL	 sCT	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that sCT inhibits gastric acid secretion via receptors localized in the hypothalamus and in adjacent areas of the brain .
	manualset3
175094	3	413613	7	NULL	NULL	0	NULL	gastric acid secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that sCT inhibits gastric acid secretion via receptors localized in the hypothalamus and in adjacent areas of the brain .
	manualset3
175095	4	413613	7	NULL	NULL	0	NULL	receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that sCT inhibits gastric acid secretion via receptors localized in the hypothalamus and in adjacent areas of the brain .
	manualset3
175096	5	413613	7	NULL	NULL	0	NULL	hypothalamus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that sCT inhibits gastric acid secretion via receptors localized in the hypothalamus and in adjacent areas of the brain .
	manualset3
175097	6	413613	7	NULL	NULL	0	NULL	adjacent areas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that sCT inhibits gastric acid secretion via receptors localized in the hypothalamus and in adjacent areas of the brain .
	manualset3
175098	7	413613	7	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that sCT inhibits gastric acid secretion via receptors localized in the hypothalamus and in adjacent areas of the brain .
	manualset3
175099	1	413614	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that the IFN-activated ISGF3 transcription factor regulates transcription through contact with DRIP150 and implicate the Mediator coactivator complex in IFN-activated gene regulation .
	manualset3
175100	2	413614	7	NULL	NULL	0	NULL	IFN-activated ISGF3 transcription factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that the IFN-activated ISGF3 transcription factor regulates transcription through contact with DRIP150 and implicate the Mediator coactivator complex in IFN-activated gene regulation .
	manualset3
175101	3	413614	7	NULL	NULL	0	NULL	transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that the IFN-activated ISGF3 transcription factor regulates transcription through contact with DRIP150 and implicate the Mediator coactivator complex in IFN-activated gene regulation .
	manualset3
175102	4	413614	7	NULL	NULL	0	NULL	DRIP150	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that the IFN-activated ISGF3 transcription factor regulates transcription through contact with DRIP150 and implicate the Mediator coactivator complex in IFN-activated gene regulation .
	manualset3
175103	5	413614	7	NULL	NULL	0	NULL	Mediator coactivator complex	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that the IFN-activated ISGF3 transcription factor regulates transcription through contact with DRIP150 and implicate the Mediator coactivator complex in IFN-activated gene regulation .
	manualset3
175104	6	413614	7	NULL	NULL	0	NULL	IFN-activated gene regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that the IFN-activated ISGF3 transcription factor regulates transcription through contact with DRIP150 and implicate the Mediator coactivator complex in IFN-activated gene regulation .
	manualset3
175105	1	413615	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that the high output of PGF2 alpha from the guinea-pig uterus during the last one-third of the oestrous cycle is not modulated by the adrenal glucocorticoid hormones .
	manualset3
175106	2	413615	7	NULL	NULL	0	NULL	 high output 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that the high output of PGF2 alpha from the guinea-pig uterus during the last one-third of the oestrous cycle is not modulated by the adrenal glucocorticoid hormones .
	manualset3
175107	3	413615	7	NULL	NULL	0	NULL	PGF2 alpha	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that the high output of PGF2 alpha from the guinea-pig uterus during the last one-third of the oestrous cycle is not modulated by the adrenal glucocorticoid hormones .
	manualset3
175108	4	413615	7	NULL	NULL	0	NULL	guinea-pig uterus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that the high output of PGF2 alpha from the guinea-pig uterus during the last one-third of the oestrous cycle is not modulated by the adrenal glucocorticoid hormones .
	manualset3
175109	5	413615	7	NULL	NULL	0	NULL	last one-third	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that the high output of PGF2 alpha from the guinea-pig uterus during the last one-third of the oestrous cycle is not modulated by the adrenal glucocorticoid hormones .
	manualset3
175110	6	413615	7	NULL	NULL	0	NULL	oestrous cycle	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that the high output of PGF2 alpha from the guinea-pig uterus during the last one-third of the oestrous cycle is not modulated by the adrenal glucocorticoid hormones .
	manualset3
175111	7	413615	7	NULL	NULL	0	NULL	 adrenal glucocorticoid hormones	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that the high output of PGF2 alpha from the guinea-pig uterus during the last one-third of the oestrous cycle is not modulated by the adrenal glucocorticoid hormones .
	manualset3
175112	1	413616	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that the riboflavin deficiency caused some defects at specific glucosensitive sites localized in the pancreas and the brain and that some metabolic processes were necessary to restore the sensitivity .
	manualset3
175113	2	413616	7	NULL	NULL	0	NULL	riboflavin deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that the riboflavin deficiency caused some defects at specific glucosensitive sites localized in the pancreas and the brain and that some metabolic processes were necessary to restore the sensitivity .
	manualset3
175114	3	413616	7	NULL	NULL	0	NULL	defects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that the riboflavin deficiency caused some defects at specific glucosensitive sites localized in the pancreas and the brain and that some metabolic processes were necessary to restore the sensitivity .
	manualset3
175115	4	413616	7	NULL	NULL	0	NULL	glucosensitive sites	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that the riboflavin deficiency caused some defects at specific glucosensitive sites localized in the pancreas and the brain and that some metabolic processes were necessary to restore the sensitivity .
	manualset3
175116	5	413616	7	NULL	NULL	0	NULL	pancreas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that the riboflavin deficiency caused some defects at specific glucosensitive sites localized in the pancreas and the brain and that some metabolic processes were necessary to restore the sensitivity .
	manualset3
175117	6	413616	7	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that the riboflavin deficiency caused some defects at specific glucosensitive sites localized in the pancreas and the brain and that some metabolic processes were necessary to restore the sensitivity .
	manualset3
175118	7	413616	7	NULL	NULL	0	NULL	metabolic processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that the riboflavin deficiency caused some defects at specific glucosensitive sites localized in the pancreas and the brain and that some metabolic processes were necessary to restore the sensitivity .
	manualset3
175119	8	413616	7	NULL	NULL	0	NULL	sensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that the riboflavin deficiency caused some defects at specific glucosensitive sites localized in the pancreas and the brain and that some metabolic processes were necessary to restore the sensitivity .
	manualset3
175120	1	413617	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that the terminal sialylation pattern of L-selectin modulates its binding characteristics .
	manualset3
175121	2	413617	7	NULL	NULL	0	NULL	 terminal sialylation pattern	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that the terminal sialylation pattern of L-selectin modulates its binding characteristics .
	manualset3
175122	3	413617	7	NULL	NULL	0	NULL	L-selectin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that the terminal sialylation pattern of L-selectin modulates its binding characteristics .
	manualset3
175123	4	413617	7	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate that the terminal sialylation pattern of L-selectin modulates its binding characteristics .
	manualset3
175124	1	413618	7	NULL	NULL	0	NULL	rosiglitazone therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Add-on rosiglitazone therapy improves plasminogen activity and high-density lipoprotein cholesterol in type 2 diabetes mellitus .
	manualset3
175125	2	413618	7	NULL	NULL	0	NULL	plasminogen activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Add-on rosiglitazone therapy improves plasminogen activity and high-density lipoprotein cholesterol in type 2 diabetes mellitus .
	manualset3
175126	3	413618	7	NULL	NULL	0	NULL	high-density lipoprotein cholesterol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Add-on rosiglitazone therapy improves plasminogen activity and high-density lipoprotein cholesterol in type 2 diabetes mellitus .
	manualset3
175127	4	413618	7	NULL	NULL	0	NULL	 type 2 diabetes mellitus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Add-on rosiglitazone therapy improves plasminogen activity and high-density lipoprotein cholesterol in type 2 diabetes mellitus .
	manualset3
175128	1	413619	7	NULL	NULL	0	NULL	 findings 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate the need to harmonize viral procedures and surveillance systems in European countries in order to improve validity and comparability of results and as a prerequisite for early information on influenza etiology and spread .
	manualset3
175129	2	413619	7	NULL	NULL	0	NULL	viral procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate the need to harmonize viral procedures and surveillance systems in European countries in order to improve validity and comparability of results and as a prerequisite for early information on influenza etiology and spread .
	manualset3
175130	3	413619	7	NULL	NULL	0	NULL	surveillance systems	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate the need to harmonize viral procedures and surveillance systems in European countries in order to improve validity and comparability of results and as a prerequisite for early information on influenza etiology and spread .
	manualset3
175131	4	413619	7	NULL	NULL	0	NULL	European countries	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate the need to harmonize viral procedures and surveillance systems in European countries in order to improve validity and comparability of results and as a prerequisite for early information on influenza etiology and spread .
	manualset3
175132	5	413619	7	NULL	NULL	0	NULL	validity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate the need to harmonize viral procedures and surveillance systems in European countries in order to improve validity and comparability of results and as a prerequisite for early information on influenza etiology and spread .
	manualset3
175133	6	413619	7	NULL	NULL	0	NULL	comparability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate the need to harmonize viral procedures and surveillance systems in European countries in order to improve validity and comparability of results and as a prerequisite for early information on influenza etiology and spread .
	manualset3
175134	7	413619	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate the need to harmonize viral procedures and surveillance systems in European countries in order to improve validity and comparability of results and as a prerequisite for early information on influenza etiology and spread .
	manualset3
175135	8	413619	7	NULL	NULL	0	NULL	early information	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate the need to harmonize viral procedures and surveillance systems in European countries in order to improve validity and comparability of results and as a prerequisite for early information on influenza etiology and spread .
	manualset3
175136	9	413619	7	NULL	NULL	0	NULL	influenza etiology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate the need to harmonize viral procedures and surveillance systems in European countries in order to improve validity and comparability of results and as a prerequisite for early information on influenza etiology and spread .
	manualset3
175137	10	413619	7	NULL	NULL	0	NULL	prerequisite 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicate the need to harmonize viral procedures and surveillance systems in European countries in order to improve validity and comparability of results and as a prerequisite for early information on influenza etiology and spread .
	manualset3
175138	1	413620	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicated the possible broader application for OPS , as they demonstrated that the physical advantages of rapid cooling and warming may be accompanied by different chemical composition ( holding media , cryoprotective additives ) according to the requirements of the biological structure .
	manualset3
175139	2	413620	7	NULL	NULL	0	NULL	application	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicated the possible broader application for OPS , as they demonstrated that the physical advantages of rapid cooling and warming may be accompanied by different chemical composition ( holding media , cryoprotective additives ) according to the requirements of the biological structure .
	manualset3
175140	3	413620	7	NULL	NULL	0	NULL	OPS	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicated the possible broader application for OPS , as they demonstrated that the physical advantages of rapid cooling and warming may be accompanied by different chemical composition ( holding media , cryoprotective additives ) according to the requirements of the biological structure .
	manualset3
175141	4	413620	7	NULL	NULL	0	NULL	physical advantages	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicated the possible broader application for OPS , as they demonstrated that the physical advantages of rapid cooling and warming may be accompanied by different chemical composition ( holding media , cryoprotective additives ) according to the requirements of the biological structure .
	manualset3
175142	5	413620	7	NULL	NULL	0	NULL	rapid cooling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicated the possible broader application for OPS , as they demonstrated that the physical advantages of rapid cooling and warming may be accompanied by different chemical composition ( holding media , cryoprotective additives ) according to the requirements of the biological structure .
	manualset3
175143	6	413620	7	NULL	NULL	0	NULL	warming	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicated the possible broader application for OPS , as they demonstrated that the physical advantages of rapid cooling and warming may be accompanied by different chemical composition ( holding media , cryoprotective additives ) according to the requirements of the biological structure .
	manualset3
175144	7	413620	7	NULL	NULL	0	NULL	chemical composition	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicated the possible broader application for OPS , as they demonstrated that the physical advantages of rapid cooling and warming may be accompanied by different chemical composition ( holding media , cryoprotective additives ) according to the requirements of the biological structure .
	manualset3
175145	8	413620	7	NULL	NULL	NULL	NULL	holding media	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings indicated the possible broader application for OPS , as they demonstrated that the physical advantages of rapid cooling and warming may be accompanied by different chemical composition ( holding media , cryoprotective additives ) according to the requirements of the biological structure .
	manualset3
175146	9	413620	7	NULL	NULL	0	NULL	cryoprotective additives	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicated the possible broader application for OPS , as they demonstrated that the physical advantages of rapid cooling and warming may be accompanied by different chemical composition ( holding media , cryoprotective additives ) according to the requirements of the biological structure .
	manualset3
175147	10	413620	7	NULL	NULL	0	NULL	 requirements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicated the possible broader application for OPS , as they demonstrated that the physical advantages of rapid cooling and warming may be accompanied by different chemical composition ( holding media , cryoprotective additives ) according to the requirements of the biological structure .
	manualset3
175148	11	413620	7	NULL	NULL	0	NULL	biological structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings indicated the possible broader application for OPS , as they demonstrated that the physical advantages of rapid cooling and warming may be accompanied by different chemical composition ( holding media , cryoprotective additives ) according to the requirements of the biological structure .
	manualset3
175149	1	413621	7	NULL	NULL	0	NULL	findings 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings may enhance our understanding of the molecular mechanism of herbicide resistance and stereochemistry-activity relationships , which may provide a new starting point for the identification of more potent inhibitors against both sensitive and resistant ACCase .
	manualset3
175150	2	413621	7	NULL	NULL	0	NULL	understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings may enhance our understanding of the molecular mechanism of herbicide resistance and stereochemistry-activity relationships , which may provide a new starting point for the identification of more potent inhibitors against both sensitive and resistant ACCase .
	manualset3
175151	3	413621	7	NULL	NULL	0	NULL	molecular mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings may enhance our understanding of the molecular mechanism of herbicide resistance and stereochemistry-activity relationships , which may provide a new starting point for the identification of more potent inhibitors against both sensitive and resistant ACCase .
	manualset3
175152	4	413621	7	NULL	NULL	NULL	NULL	herbicide resistance	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings may enhance our understanding of the molecular mechanism of herbicide resistance and stereochemistry-activity relationships , which may provide a new starting point for the identification of more potent inhibitors against both sensitive and resistant ACCase .
	manualset3
175153	5	413621	7	NULL	NULL	0	NULL	stereochemistry-activity relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings may enhance our understanding of the molecular mechanism of herbicide resistance and stereochemistry-activity relationships , which may provide a new starting point for the identification of more potent inhibitors against both sensitive and resistant ACCase .
	manualset3
175154	6	413621	7	NULL	NULL	0	NULL	starting point	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings may enhance our understanding of the molecular mechanism of herbicide resistance and stereochemistry-activity relationships , which may provide a new starting point for the identification of more potent inhibitors against both sensitive and resistant ACCase .
	manualset3
175155	7	413621	7	NULL	NULL	0	NULL	identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings may enhance our understanding of the molecular mechanism of herbicide resistance and stereochemistry-activity relationships , which may provide a new starting point for the identification of more potent inhibitors against both sensitive and resistant ACCase .
	manualset3
175156	8	413621	7	NULL	NULL	0	NULL	potent inhibitors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings may enhance our understanding of the molecular mechanism of herbicide resistance and stereochemistry-activity relationships , which may provide a new starting point for the identification of more potent inhibitors against both sensitive and resistant ACCase .
	manualset3
175157	9	413621	7	NULL	NULL	0	NULL	ACCase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings may enhance our understanding of the molecular mechanism of herbicide resistance and stereochemistry-activity relationships , which may provide a new starting point for the identification of more potent inhibitors against both sensitive and resistant ACCase .
	manualset3
175158	1	413622	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings may inform studies investigating mechanisms that regulate progenitor cell recruitment in disease and can be exploited to provide efficacious stem cell therapy for tissue regeneration .
	manualset3
175159	2	413622	7	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings may inform studies investigating mechanisms that regulate progenitor cell recruitment in disease and can be exploited to provide efficacious stem cell therapy for tissue regeneration .
	manualset3
175160	3	413622	7	NULL	NULL	0	NULL	mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings may inform studies investigating mechanisms that regulate progenitor cell recruitment in disease and can be exploited to provide efficacious stem cell therapy for tissue regeneration .
	manualset3
175161	4	413622	7	NULL	NULL	0	NULL	progenitor cell recruitment 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings may inform studies investigating mechanisms that regulate progenitor cell recruitment in disease and can be exploited to provide efficacious stem cell therapy for tissue regeneration .
	manualset3
175162	5	413622	7	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings may inform studies investigating mechanisms that regulate progenitor cell recruitment in disease and can be exploited to provide efficacious stem cell therapy for tissue regeneration .
	manualset3
175163	6	413622	7	NULL	NULL	0	NULL	stem cell therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings may inform studies investigating mechanisms that regulate progenitor cell recruitment in disease and can be exploited to provide efficacious stem cell therapy for tissue regeneration .
	manualset3
175164	7	413622	7	NULL	NULL	0	NULL	tissue regeneration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings may inform studies investigating mechanisms that regulate progenitor cell recruitment in disease and can be exploited to provide efficacious stem cell therapy for tissue regeneration .
	manualset3
175165	1	413623	7	NULL	NULL	0	NULL	 findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings point to the normal function of the central conductive pathways .
	manualset3
175166	2	413623	7	NULL	NULL	0	NULL	normal function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings point to the normal function of the central conductive pathways .
	manualset3
175167	3	413623	7	NULL	NULL	0	NULL	central conductive pathways	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings point to the normal function of the central conductive pathways .
	manualset3
175168	1	413624	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings propose standardized measures that may be useful in assessing the beliefs and attitudes of gay men toward HBV vaccination to guide intervention design and evaluation .
	manualset3
175169	2	413624	7	NULL	NULL	NULL	NULL	standardized measures	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings propose standardized measures that may be useful in assessing the beliefs and attitudes of gay men toward HBV vaccination to guide intervention design and evaluation .
	manualset3
175170	3	413624	7	NULL	NULL	0	NULL	beliefs 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings propose standardized measures that may be useful in assessing the beliefs and attitudes of gay men toward HBV vaccination to guide intervention design and evaluation .
	manualset3
175171	4	413624	7	NULL	NULL	0	NULL	attitudes 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings propose standardized measures that may be useful in assessing the beliefs and attitudes of gay men toward HBV vaccination to guide intervention design and evaluation .
	manualset3
175172	5	413624	7	NULL	NULL	0	NULL	gay men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings propose standardized measures that may be useful in assessing the beliefs and attitudes of gay men toward HBV vaccination to guide intervention design and evaluation .
	manualset3
175173	6	413624	7	NULL	NULL	0	NULL	HBV vaccination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings propose standardized measures that may be useful in assessing the beliefs and attitudes of gay men toward HBV vaccination to guide intervention design and evaluation .
	manualset3
175174	7	413624	7	NULL	NULL	0	NULL	intervention design	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings propose standardized measures that may be useful in assessing the beliefs and attitudes of gay men toward HBV vaccination to guide intervention design and evaluation .
	manualset3
175175	8	413624	7	NULL	NULL	0	NULL	evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings propose standardized measures that may be useful in assessing the beliefs and attitudes of gay men toward HBV vaccination to guide intervention design and evaluation .
	manualset3
175176	1	413625	7	NULL	NULL	0	NULL	Addictive genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Addictive genes and the relationship to obesity and inflammation .
	manualset3
175177	2	413625	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Addictive genes and the relationship to obesity and inflammation .
	manualset3
175178	3	413625	7	NULL	NULL	0	NULL	obesity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Addictive genes and the relationship to obesity and inflammation .
	manualset3
175179	4	413625	7	NULL	NULL	0	NULL	inflammation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Addictive genes and the relationship to obesity and inflammation .
	manualset3
175180	1	413626	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings provide further evidence of neurochemical heterogeneity in the striatum .
	manualset3
175181	2	413626	7	NULL	NULL	0	NULL	evidence 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings provide further evidence of neurochemical heterogeneity in the striatum .
	manualset3
175182	3	413626	7	NULL	NULL	0	NULL	neurochemical heterogeneity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings provide further evidence of neurochemical heterogeneity in the striatum .
	manualset3
175183	4	413626	7	NULL	NULL	0	NULL	striatum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings provide further evidence of neurochemical heterogeneity in the striatum .
	manualset3
175184	1	413627	7	NULL	NULL	0	NULL	 findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings provide insight to suicide resilience profiles across and within ethnic groups and suggest that assessments of reasons for living and cultural correlates might have important implications for future research and clinical practice .
	manualset3
175185	2	413627	7	NULL	NULL	0	NULL	suicide resilience profiles	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings provide insight to suicide resilience profiles across and within ethnic groups and suggest that assessments of reasons for living and cultural correlates might have important implications for future research and clinical practice .
	manualset3
175186	3	413627	7	NULL	NULL	0	NULL	ethnic groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings provide insight to suicide resilience profiles across and within ethnic groups and suggest that assessments of reasons for living and cultural correlates might have important implications for future research and clinical practice .
	manualset3
175187	4	413627	7	NULL	NULL	0	NULL	assessments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings provide insight to suicide resilience profiles across and within ethnic groups and suggest that assessments of reasons for living and cultural correlates might have important implications for future research and clinical practice .
	manualset3
175188	5	413627	7	NULL	NULL	0	NULL	reasons	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings provide insight to suicide resilience profiles across and within ethnic groups and suggest that assessments of reasons for living and cultural correlates might have important implications for future research and clinical practice .
	manualset3
175189	6	413627	7	NULL	NULL	0	NULL	living	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings provide insight to suicide resilience profiles across and within ethnic groups and suggest that assessments of reasons for living and cultural correlates might have important implications for future research and clinical practice .
	manualset3
175190	7	413627	7	NULL	NULL	0	NULL	implications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings provide insight to suicide resilience profiles across and within ethnic groups and suggest that assessments of reasons for living and cultural correlates might have important implications for future research and clinical practice .
	manualset3
175191	8	413627	7	NULL	NULL	0	NULL	future research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings provide insight to suicide resilience profiles across and within ethnic groups and suggest that assessments of reasons for living and cultural correlates might have important implications for future research and clinical practice .
	manualset3
175192	9	413627	7	NULL	NULL	0	NULL	clinical practice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings provide insight to suicide resilience profiles across and within ethnic groups and suggest that assessments of reasons for living and cultural correlates might have important implications for future research and clinical practice .
	manualset3
175193	1	413628	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings provide mechanistic insights into the metastatic process and have implications about the importance of pleiotropy for the biological actions of miRNAs .
	manualset3
175194	2	413628	7	NULL	NULL	0	NULL	mechanistic insights	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings provide mechanistic insights into the metastatic process and have implications about the importance of pleiotropy for the biological actions of miRNAs .
	manualset3
175195	3	413628	7	NULL	NULL	0	NULL	metastatic process	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings provide mechanistic insights into the metastatic process and have implications about the importance of pleiotropy for the biological actions of miRNAs .
	manualset3
175196	4	413628	7	NULL	NULL	0	NULL	implications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings provide mechanistic insights into the metastatic process and have implications about the importance of pleiotropy for the biological actions of miRNAs .
	manualset3
175197	5	413628	7	NULL	NULL	0	NULL	 pleiotropy 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings provide mechanistic insights into the metastatic process and have implications about the importance of pleiotropy for the biological actions of miRNAs .
	manualset3
175198	6	413628	7	NULL	NULL	NULL	NULL	biological actions	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings provide mechanistic insights into the metastatic process and have implications about the importance of pleiotropy for the biological actions of miRNAs .
	manualset3
175199	7	413628	7	NULL	NULL	0	NULL	miRNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings provide mechanistic insights into the metastatic process and have implications about the importance of pleiotropy for the biological actions of miRNAs .
	manualset3
175200	1	413629	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings question the need for corticosteroid `` cover '' for the stress of surgery in patients who have been taking corticosteroid drugs .
	manualset3
175201	2	413629	7	NULL	NULL	0	NULL	need 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings question the need for corticosteroid `` cover '' for the stress of surgery in patients who have been taking corticosteroid drugs .
	manualset3
175202	3	413629	7	NULL	NULL	0	NULL	corticosteroid `` cover '	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings question the need for corticosteroid `` cover '' for the stress of surgery in patients who have been taking corticosteroid drugs .
	manualset3
175203	4	413629	7	NULL	NULL	0	NULL	stress	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings question the need for corticosteroid `` cover '' for the stress of surgery in patients who have been taking corticosteroid drugs .
	manualset3
175204	5	413629	7	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings question the need for corticosteroid `` cover '' for the stress of surgery in patients who have been taking corticosteroid drugs .
	manualset3
175205	6	413629	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings question the need for corticosteroid `` cover '' for the stress of surgery in patients who have been taking corticosteroid drugs .
	manualset3
175206	7	413629	7	NULL	NULL	0	NULL	corticosteroid drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings question the need for corticosteroid `` cover '' for the stress of surgery in patients who have been taking corticosteroid drugs .
	manualset3
175207	1	413630	7	NULL	NULL	0	NULL	findings 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings represent reversible qualitative changes produced by a hormone in the target tissue .
	manualset3
175208	2	413630	7	NULL	NULL	0	NULL	reversible qualitative changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings represent reversible qualitative changes produced by a hormone in the target tissue .
	manualset3
175209	3	413630	7	NULL	NULL	0	NULL	hormone 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings represent reversible qualitative changes produced by a hormone in the target tissue .
	manualset3
175210	4	413630	7	NULL	NULL	0	NULL	 target tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings represent reversible qualitative changes produced by a hormone in the target tissue .
	manualset3
175334	1	413631	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings revealed that S1P ( 1 ) is a critical component of VEGF-related angiogenic responses and also provide evidence for the efficacy of TASP0277308 for anti-cancer therapies .
	manualset3
175335	2	413631	7	NULL	NULL	0	NULL	 S1P ( 1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings revealed that S1P ( 1 ) is a critical component of VEGF-related angiogenic responses and also provide evidence for the efficacy of TASP0277308 for anti-cancer therapies .
	manualset3
175336	3	413631	7	NULL	NULL	0	NULL	VEGF-related angiogenic responses	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings revealed that S1P ( 1 ) is a critical component of VEGF-related angiogenic responses and also provide evidence for the efficacy of TASP0277308 for anti-cancer therapies .
	manualset3
175337	4	413631	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings revealed that S1P ( 1 ) is a critical component of VEGF-related angiogenic responses and also provide evidence for the efficacy of TASP0277308 for anti-cancer therapies .
	manualset3
175338	5	413631	7	NULL	NULL	0	NULL	 efficacy	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings revealed that S1P ( 1 ) is a critical component of VEGF-related angiogenic responses and also provide evidence for the efficacy of TASP0277308 for anti-cancer therapies .
	manualset3
175339	6	413631	7	NULL	NULL	0	NULL	TASP0277308	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings revealed that S1P ( 1 ) is a critical component of VEGF-related angiogenic responses and also provide evidence for the efficacy of TASP0277308 for anti-cancer therapies .
	manualset3
175340	7	413631	7	NULL	NULL	0	NULL	anti-cancer therapies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings revealed that S1P ( 1 ) is a critical component of VEGF-related angiogenic responses and also provide evidence for the efficacy of TASP0277308 for anti-cancer therapies .
	manualset3
175341	8	413631	7	NULL	NULL	0	NULL	critical component	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings revealed that S1P ( 1 ) is a critical component of VEGF-related angiogenic responses and also provide evidence for the efficacy of TASP0277308 for anti-cancer therapies .
	manualset3
175342	1	413632	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings show that H-bonding to the C-13 ( 1 ) keto group ofbeta-ligated ( bacterio ) - chlorophyll is a key structural motif and significantly contributes to the stability of bacteriochlorophyll proteins in the native membrane .
	manualset3
175343	2	413632	7	NULL	NULL	0	NULL	H-bonding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings show that H-bonding to the C-13 ( 1 ) keto group ofbeta-ligated ( bacterio ) - chlorophyll is a key structural motif and significantly contributes to the stability of bacteriochlorophyll proteins in the native membrane .
	manualset3
175344	3	413632	7	NULL	NULL	NULL	NULL	C-13 ( 1 ) keto group	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings show that H-bonding to the C-13 ( 1 ) keto group ofbeta-ligated ( bacterio ) - chlorophyll is a key structural motif and significantly contributes to the stability of bacteriochlorophyll proteins in the native membrane .
	manualset3
175345	4	413632	7	NULL	NULL	0	NULL	beta-ligated ( bacterio ) - chlorophyll	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings show that H-bonding to the C-13 ( 1 ) keto group ofbeta-ligated ( bacterio ) - chlorophyll is a key structural motif and significantly contributes to the stability of bacteriochlorophyll proteins in the native membrane .
	manualset3
175346	5	413632	7	NULL	NULL	NULL	NULL	structural motif	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings show that H-bonding to the C-13 ( 1 ) keto group ofbeta-ligated ( bacterio ) - chlorophyll is a key structural motif and significantly contributes to the stability of bacteriochlorophyll proteins in the native membrane .
	manualset3
175347	6	413632	7	NULL	NULL	0	NULL	stability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings show that H-bonding to the C-13 ( 1 ) keto group ofbeta-ligated ( bacterio ) - chlorophyll is a key structural motif and significantly contributes to the stability of bacteriochlorophyll proteins in the native membrane .
	manualset3
175348	7	413632	7	NULL	NULL	NULL	NULL	bacteriochlorophyll proteins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings show that H-bonding to the C-13 ( 1 ) keto group ofbeta-ligated ( bacterio ) - chlorophyll is a key structural motif and significantly contributes to the stability of bacteriochlorophyll proteins in the native membrane .
	manualset3
175349	8	413632	7	NULL	NULL	0	NULL	native membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings show that H-bonding to the C-13 ( 1 ) keto group ofbeta-ligated ( bacterio ) - chlorophyll is a key structural motif and significantly contributes to the stability of bacteriochlorophyll proteins in the native membrane .
	manualset3
175356	1	413633	7	NULL	NULL	0	NULL	 findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings signify that 1b micelles may be a promising carrier for delivery of anticancer drugs that contain amine groups .
	manualset3
175358	2	413633	7	NULL	NULL	0	NULL	1b micelles	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings signify that 1b micelles may be a promising carrier for delivery of anticancer drugs that contain amine groups .
	manualset3
175359	3	413633	7	NULL	NULL	NULL	NULL	carrier	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings signify that 1b micelles may be a promising carrier for delivery of anticancer drugs that contain amine groups .
	manualset3
175360	4	413633	7	NULL	NULL	NULL	NULL	delivery 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings signify that 1b micelles may be a promising carrier for delivery of anticancer drugs that contain amine groups .
	manualset3
175363	5	413633	7	NULL	NULL	0	NULL	anticancer drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings signify that 1b micelles may be a promising carrier for delivery of anticancer drugs that contain amine groups .
	manualset3
175365	6	413633	7	NULL	NULL	NULL	NULL	amine groups 	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings signify that 1b micelles may be a promising carrier for delivery of anticancer drugs that contain amine groups .
	manualset3
175371	1	413634	7	NULL	NULL	0	NULL	 findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest a possible role for ASN in MND ; however , the precise nature of this association is unclear .
	manualset3
175372	2	413634	7	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest a possible role for ASN in MND ; however , the precise nature of this association is unclear .
	manualset3
175374	3	413634	7	NULL	NULL	0	NULL	ASN	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest a possible role for ASN in MND ; however , the precise nature of this association is unclear .
	manualset3
175375	4	413634	7	NULL	NULL	0	NULL	MND	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest a possible role for ASN in MND ; however , the precise nature of this association is unclear .
	manualset3
175378	5	413634	7	NULL	NULL	0	NULL	nature 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest a possible role for ASN in MND ; however , the precise nature of this association is unclear .
	manualset3
175381	6	413634	7	NULL	NULL	0	NULL	association 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest a possible role for ASN in MND ; however , the precise nature of this association is unclear .
	manualset3
175407	1	413635	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that , in an anxiety state , reduced cognitive-behavioral flexibility may stem from enhanced stimulus-driven attention , which may serve the adaptive function of optimizing threat detection .
	manualset3
175408	2	413635	7	NULL	NULL	0	NULL	anxiety state	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that , in an anxiety state , reduced cognitive-behavioral flexibility may stem from enhanced stimulus-driven attention , which may serve the adaptive function of optimizing threat detection .
	manualset3
175409	3	413635	7	NULL	NULL	0	NULL	cognitive-behavioral flexibility 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that , in an anxiety state , reduced cognitive-behavioral flexibility may stem from enhanced stimulus-driven attention , which may serve the adaptive function of optimizing threat detection .
	manualset3
175410	4	413635	7	NULL	NULL	0	NULL	stimulus-driven attention	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that , in an anxiety state , reduced cognitive-behavioral flexibility may stem from enhanced stimulus-driven attention , which may serve the adaptive function of optimizing threat detection .
	manualset3
175412	5	413635	7	NULL	NULL	0	NULL	adaptive function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that , in an anxiety state , reduced cognitive-behavioral flexibility may stem from enhanced stimulus-driven attention , which may serve the adaptive function of optimizing threat detection .
	manualset3
175413	6	413635	7	NULL	NULL	NULL	NULL	optimizing threat detection	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings suggest that , in an anxiety state , reduced cognitive-behavioral flexibility may stem from enhanced stimulus-driven attention , which may serve the adaptive function of optimizing threat detection .
	manualset3
175418	1	413636	7	NULL	NULL	NULL	NULL	Addition	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Addition of 3 ' - phosphoadenosine 5 ' - phosphosulfate and to a lesser extent acetyl coenzyme A to cytosolic incubations also increased the rate of degradation of the unstable N-hydroxy-PhIP intermediate .
	manualset3
175419	2	413636	7	NULL	NULL	0	NULL	3 ' - phosphoadenosine 5 ' - phosphosulfate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of 3 ' - phosphoadenosine 5 ' - phosphosulfate and to a lesser extent acetyl coenzyme A to cytosolic incubations also increased the rate of degradation of the unstable N-hydroxy-PhIP intermediate .
	manualset3
175421	3	413636	7	NULL	NULL	0	NULL	acetyl coenzyme A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of 3 ' - phosphoadenosine 5 ' - phosphosulfate and to a lesser extent acetyl coenzyme A to cytosolic incubations also increased the rate of degradation of the unstable N-hydroxy-PhIP intermediate .
	manualset3
175423	4	413636	7	NULL	NULL	0	NULL	cytosolic incubations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of 3 ' - phosphoadenosine 5 ' - phosphosulfate and to a lesser extent acetyl coenzyme A to cytosolic incubations also increased the rate of degradation of the unstable N-hydroxy-PhIP intermediate .
	manualset3
175426	5	413636	7	NULL	NULL	0	NULL	rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of 3 ' - phosphoadenosine 5 ' - phosphosulfate and to a lesser extent acetyl coenzyme A to cytosolic incubations also increased the rate of degradation of the unstable N-hydroxy-PhIP intermediate .
	manualset3
175427	6	413636	7	NULL	NULL	0	NULL	degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of 3 ' - phosphoadenosine 5 ' - phosphosulfate and to a lesser extent acetyl coenzyme A to cytosolic incubations also increased the rate of degradation of the unstable N-hydroxy-PhIP intermediate .
	manualset3
175428	7	413636	7	NULL	NULL	0	NULL	 unstable N-hydroxy-PhIP intermediate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of 3 ' - phosphoadenosine 5 ' - phosphosulfate and to a lesser extent acetyl coenzyme A to cytosolic incubations also increased the rate of degradation of the unstable N-hydroxy-PhIP intermediate .
	manualset3
175440	1	413637	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that , in general , adolescents with a chronic illness cope effectively with their disability but that parents and clinicians must be sensitive to the adolescents ' feelings and concerns regarding their health and its impact on the family .
	manualset3
175443	2	413637	7	NULL	NULL	0	NULL	 adolescents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that , in general , adolescents with a chronic illness cope effectively with their disability but that parents and clinicians must be sensitive to the adolescents ' feelings and concerns regarding their health and its impact on the family .
	manualset3
175446	3	413637	7	NULL	NULL	0	NULL	chronic illness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that , in general , adolescents with a chronic illness cope effectively with their disability but that parents and clinicians must be sensitive to the adolescents ' feelings and concerns regarding their health and its impact on the family .
	manualset3
175634	4	413637	7	NULL	NULL	0	NULL	disability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that , in general , adolescents with a chronic illness cope effectively with their disability but that parents and clinicians must be sensitive to the adolescents ' feelings and concerns regarding their health and its impact on the family .
	manualset3
175635	5	413637	7	NULL	NULL	0	NULL	parents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that , in general , adolescents with a chronic illness cope effectively with their disability but that parents and clinicians must be sensitive to the adolescents ' feelings and concerns regarding their health and its impact on the family .
	manualset3
175636	6	413637	7	NULL	NULL	0	NULL	clinicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that , in general , adolescents with a chronic illness cope effectively with their disability but that parents and clinicians must be sensitive to the adolescents ' feelings and concerns regarding their health and its impact on the family .
	manualset3
175637	7	413637	7	NULL	NULL	NULL	NULL	adolescents  ' feelings 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings suggest that , in general , adolescents with a chronic illness cope effectively with their disability but that parents and clinicians must be sensitive to the adolescents ' feelings and concerns regarding their health and its impact on the family .
	manualset3
175639	9	413637	7	NULL	NULL	0	NULL	concerns	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that , in general , adolescents with a chronic illness cope effectively with their disability but that parents and clinicians must be sensitive to the adolescents ' feelings and concerns regarding their health and its impact on the family .
	manualset3
175640	10	413637	7	NULL	NULL	0	NULL	 health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that , in general , adolescents with a chronic illness cope effectively with their disability but that parents and clinicians must be sensitive to the adolescents ' feelings and concerns regarding their health and its impact on the family .
	manualset3
175641	11	413637	7	NULL	NULL	0	NULL	impact	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that , in general , adolescents with a chronic illness cope effectively with their disability but that parents and clinicians must be sensitive to the adolescents ' feelings and concerns regarding their health and its impact on the family .
	manualset3
175642	12	413637	7	NULL	NULL	0	NULL	family	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that , in general , adolescents with a chronic illness cope effectively with their disability but that parents and clinicians must be sensitive to the adolescents ' feelings and concerns regarding their health and its impact on the family .
	manualset3
175643	1	413638	7	NULL	NULL	0	NULL	 findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that 1 g of cefotetan administered before abdominal surgery would result in intraperitoneal cefotetan levels necessary to inhibit susceptible pathogens for 5 h or more .
	manualset3
175644	2	413638	7	NULL	NULL	0	NULL	1 g	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that 1 g of cefotetan administered before abdominal surgery would result in intraperitoneal cefotetan levels necessary to inhibit susceptible pathogens for 5 h or more .
	manualset3
175645	3	413638	7	NULL	NULL	0	NULL	cefotetan	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that 1 g of cefotetan administered before abdominal surgery would result in intraperitoneal cefotetan levels necessary to inhibit susceptible pathogens for 5 h or more .
	manualset3
175646	4	413638	7	NULL	NULL	0	NULL	abdominal surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that 1 g of cefotetan administered before abdominal surgery would result in intraperitoneal cefotetan levels necessary to inhibit susceptible pathogens for 5 h or more .
	manualset3
175647	5	413638	7	NULL	NULL	0	NULL	intraperitoneal cefotetan levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that 1 g of cefotetan administered before abdominal surgery would result in intraperitoneal cefotetan levels necessary to inhibit susceptible pathogens for 5 h or more .
	manualset3
175648	6	413638	7	NULL	NULL	0	NULL	susceptible pathogens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that 1 g of cefotetan administered before abdominal surgery would result in intraperitoneal cefotetan levels necessary to inhibit susceptible pathogens for 5 h or more .
	manualset3
175649	7	413638	7	NULL	NULL	0	NULL	5 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that 1 g of cefotetan administered before abdominal surgery would result in intraperitoneal cefotetan levels necessary to inhibit susceptible pathogens for 5 h or more .
	manualset3
175650	1	413639	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that Cu/Zn ratio may be used as a diagnostic test in lung cancer patients .
	manualset3
175651	2	413639	7	NULL	NULL	0	NULL	Cu/Zn ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that Cu/Zn ratio may be used as a diagnostic test in lung cancer patients .
	manualset3
175652	3	413639	7	NULL	NULL	0	NULL	diagnostic test	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that Cu/Zn ratio may be used as a diagnostic test in lung cancer patients .
	manualset3
175653	4	413639	7	NULL	NULL	0	NULL	lung cancer patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that Cu/Zn ratio may be used as a diagnostic test in lung cancer patients .
	manualset3
175654	1	413640	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that FAK functions in the regulation of cell migration and cell proliferation .
	manualset3
175655	2	413640	7	NULL	NULL	0	NULL	FAK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that FAK functions in the regulation of cell migration and cell proliferation .
	manualset3
175656	3	413640	7	NULL	NULL	0	NULL	 regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that FAK functions in the regulation of cell migration and cell proliferation .
	manualset3
175657	4	413640	7	NULL	NULL	0	NULL	cell migration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that FAK functions in the regulation of cell migration and cell proliferation .
	manualset3
175658	5	413640	7	NULL	NULL	0	NULL	cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that FAK functions in the regulation of cell migration and cell proliferation .
	manualset3
175659	1	413641	7	NULL	NULL	0	NULL	 findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that H2O2 and vanadate interact with the protein tyrosine phosphatases at two independent sites .
	manualset3
175660	2	413641	7	NULL	NULL	0	NULL	H2O2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that H2O2 and vanadate interact with the protein tyrosine phosphatases at two independent sites .
	manualset3
175661	3	413641	7	NULL	NULL	0	NULL	vanadate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that H2O2 and vanadate interact with the protein tyrosine phosphatases at two independent sites .
	manualset3
175662	4	413641	7	NULL	NULL	0	NULL	protein tyrosine phosphatases	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that H2O2 and vanadate interact with the protein tyrosine phosphatases at two independent sites .
	manualset3
175663	5	413641	7	NULL	NULL	0	NULL	two independent sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that H2O2 and vanadate interact with the protein tyrosine phosphatases at two independent sites .
	manualset3
175664	1	413642	7	NULL	NULL	0	NULL	 findings 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that HMGB1 released by AA-injured hepatocytes contributes to macrophage activation .
	manualset3
175665	2	413642	7	NULL	NULL	0	NULL	HMGB1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that HMGB1 released by AA-injured hepatocytes contributes to macrophage activation .
	manualset3
175666	3	413642	7	NULL	NULL	0	NULL	AA-injured hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that HMGB1 released by AA-injured hepatocytes contributes to macrophage activation .
	manualset3
175667	4	413642	7	NULL	NULL	0	NULL	 macrophage activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that HMGB1 released by AA-injured hepatocytes contributes to macrophage activation .
	manualset3
175668	1	413643	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that JNK phosphorylation is closely associated with the clearance of inflammatory cells as well as the activation of Schwann cells in the EAN affected sciatic nerves .
	manualset3
175669	2	413643	7	NULL	NULL	0	NULL	 JNK phosphorylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that JNK phosphorylation is closely associated with the clearance of inflammatory cells as well as the activation of Schwann cells in the EAN affected sciatic nerves .
	manualset3
175670	3	413643	7	NULL	NULL	0	NULL	clearance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that JNK phosphorylation is closely associated with the clearance of inflammatory cells as well as the activation of Schwann cells in the EAN affected sciatic nerves .
	manualset3
175671	4	413643	7	NULL	NULL	0	NULL	inflammatory cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that JNK phosphorylation is closely associated with the clearance of inflammatory cells as well as the activation of Schwann cells in the EAN affected sciatic nerves .
	manualset3
175672	5	413643	7	NULL	NULL	0	NULL	activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that JNK phosphorylation is closely associated with the clearance of inflammatory cells as well as the activation of Schwann cells in the EAN affected sciatic nerves .
	manualset3
175673	6	413643	7	NULL	NULL	0	NULL	Schwann cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that JNK phosphorylation is closely associated with the clearance of inflammatory cells as well as the activation of Schwann cells in the EAN affected sciatic nerves .
	manualset3
175674	7	413643	7	NULL	NULL	0	NULL	EAN affected sciatic nerves	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that JNK phosphorylation is closely associated with the clearance of inflammatory cells as well as the activation of Schwann cells in the EAN affected sciatic nerves .
	manualset3
175677	1	413644	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that a localized immunosuppression associated with the rise in the Ly-2 + cells may be of functional significance during carcinogen-induced tumor development .
	manualset3
175678	2	413644	7	NULL	NULL	0	NULL	 localized immunosuppression 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that a localized immunosuppression associated with the rise in the Ly-2 + cells may be of functional significance during carcinogen-induced tumor development .
	manualset3
175679	3	413644	7	NULL	NULL	0	NULL	 rise	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that a localized immunosuppression associated with the rise in the Ly-2 + cells may be of functional significance during carcinogen-induced tumor development .
	manualset3
175680	4	413644	7	NULL	NULL	0	NULL	Ly-2 + cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that a localized immunosuppression associated with the rise in the Ly-2 + cells may be of functional significance during carcinogen-induced tumor development .
	manualset3
175681	5	413644	7	NULL	NULL	0	NULL	carcinogen-induced tumor development	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that a localized immunosuppression associated with the rise in the Ly-2 + cells may be of functional significance during carcinogen-induced tumor development .
	manualset3
175682	1	413645	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that an awareness of SIADH and avoiding intravenous fluid overloads by accurately managing intraoperative and postoperative fluids will decrease the dilutional effects observed on blood indices and perhaps save patients from unwarranted transfusions .
	manualset3
175683	2	413645	7	NULL	NULL	0	NULL	awareness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that an awareness of SIADH and avoiding intravenous fluid overloads by accurately managing intraoperative and postoperative fluids will decrease the dilutional effects observed on blood indices and perhaps save patients from unwarranted transfusions .
	manualset3
175684	3	413645	7	NULL	NULL	0	NULL	SIADH	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that an awareness of SIADH and avoiding intravenous fluid overloads by accurately managing intraoperative and postoperative fluids will decrease the dilutional effects observed on blood indices and perhaps save patients from unwarranted transfusions .
	manualset3
175685	4	413645	7	NULL	NULL	0	NULL	intravenous fluid	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that an awareness of SIADH and avoiding intravenous fluid overloads by accurately managing intraoperative and postoperative fluids will decrease the dilutional effects observed on blood indices and perhaps save patients from unwarranted transfusions .
	manualset3
175686	5	413645	7	NULL	NULL	0	NULL	 intraoperative fluids	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that an awareness of SIADH and avoiding intravenous fluid overloads by accurately managing intraoperative and postoperative fluids will decrease the dilutional effects observed on blood indices and perhaps save patients from unwarranted transfusions .
	manualset3
175687	6	413645	7	NULL	NULL	0	NULL	postoperative fluids	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that an awareness of SIADH and avoiding intravenous fluid overloads by accurately managing intraoperative and postoperative fluids will decrease the dilutional effects observed on blood indices and perhaps save patients from unwarranted transfusions .
	manualset3
175688	7	413645	7	NULL	NULL	0	NULL	dilutional effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that an awareness of SIADH and avoiding intravenous fluid overloads by accurately managing intraoperative and postoperative fluids will decrease the dilutional effects observed on blood indices and perhaps save patients from unwarranted transfusions .
	manualset3
175689	8	413645	7	NULL	NULL	0	NULL	blood indices	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that an awareness of SIADH and avoiding intravenous fluid overloads by accurately managing intraoperative and postoperative fluids will decrease the dilutional effects observed on blood indices and perhaps save patients from unwarranted transfusions .
	manualset3
175690	9	413645	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that an awareness of SIADH and avoiding intravenous fluid overloads by accurately managing intraoperative and postoperative fluids will decrease the dilutional effects observed on blood indices and perhaps save patients from unwarranted transfusions .
	manualset3
175691	10	413645	7	NULL	NULL	NULL	NULL	unwarranted transfusions	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings suggest that an awareness of SIADH and avoiding intravenous fluid overloads by accurately managing intraoperative and postoperative fluids will decrease the dilutional effects observed on blood indices and perhaps save patients from unwarranted transfusions .
	manualset3
175729	1	413646	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that cAMP plays a key role in K ( ATP ) - independent insulin secretion and that the GLP-1 receptor is constitutively active in SUR-1 ( - / - ) beta-cells .
	manualset3
175730	2	413646	7	NULL	NULL	0	NULL	cAMP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that cAMP plays a key role in K ( ATP ) - independent insulin secretion and that the GLP-1 receptor is constitutively active in SUR-1 ( - / - ) beta-cells .
	manualset3
175731	3	413646	7	NULL	NULL	0	NULL	 role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that cAMP plays a key role in K ( ATP ) - independent insulin secretion and that the GLP-1 receptor is constitutively active in SUR-1 ( - / - ) beta-cells .
	manualset3
175732	4	413646	7	NULL	NULL	0	NULL	K ( ATP ) - independent insulin secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that cAMP plays a key role in K ( ATP ) - independent insulin secretion and that the GLP-1 receptor is constitutively active in SUR-1 ( - / - ) beta-cells .
	manualset3
175733	5	413646	7	NULL	NULL	0	NULL	GLP-1 receptor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that cAMP plays a key role in K ( ATP ) - independent insulin secretion and that the GLP-1 receptor is constitutively active in SUR-1 ( - / - ) beta-cells .
	manualset3
175734	6	413646	7	NULL	NULL	0	NULL	SUR-1 ( - / - ) beta-cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that cAMP plays a key role in K ( ATP ) - independent insulin secretion and that the GLP-1 receptor is constitutively active in SUR-1 ( - / - ) beta-cells .
	manualset3
175735	1	413647	7	NULL	NULL	NULL	NULL	SLE ACS	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Addition of SLE ACS to cultures of normal mononuclear cells did not stimulate ISC production .
	manualset3
175737	2	413647	7	NULL	NULL	0	NULL	normal mononuclear cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of SLE ACS to cultures of normal mononuclear cells did not stimulate ISC production .
	manualset3
175740	3	413647	7	NULL	NULL	0	NULL	 ISC production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of SLE ACS to cultures of normal mononuclear cells did not stimulate ISC production .
	manualset3
175742	4	413647	7	NULL	NULL	0	NULL	cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of SLE ACS to cultures of normal mononuclear cells did not stimulate ISC production .
	manualset3
178198	5	413647	7	NULL	NULL	0	NULL	Addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of SLE ACS to cultures of normal mononuclear cells did not stimulate ISC production .
	manualset3
175743	1	413648	7	NULL	NULL	0	NULL	 findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that humoral immunity as well as cellular immunity may play a part in the production of the rash .
	manualset3
175750	2	413648	7	NULL	NULL	0	NULL	humoral immunity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that humoral immunity as well as cellular immunity may play a part in the production of the rash .
	manualset3
175751	3	413648	7	NULL	NULL	0	NULL	 cellular immunity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that humoral immunity as well as cellular immunity may play a part in the production of the rash .
	manualset3
175752	4	413648	7	NULL	NULL	0	NULL	part	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that humoral immunity as well as cellular immunity may play a part in the production of the rash .
	manualset3
175754	5	413648	7	NULL	NULL	0	NULL	production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that humoral immunity as well as cellular immunity may play a part in the production of the rash .
	manualset3
175757	6	413648	7	NULL	NULL	0	NULL	rash	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that humoral immunity as well as cellular immunity may play a part in the production of the rash .
	manualset3
175761	1	413649	7	NULL	NULL	0	NULL	 findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that in human dermal fibroblasts , Akt has dual profibrotic effects , increasing collagen synthesis and decreasing its degradation via downregulation of MMP1 .
	manualset3
175762	2	413649	7	NULL	NULL	0	NULL	human dermal fibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that in human dermal fibroblasts , Akt has dual profibrotic effects , increasing collagen synthesis and decreasing its degradation via downregulation of MMP1 .
	manualset3
175763	3	413649	7	NULL	NULL	0	NULL	Akt 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that in human dermal fibroblasts , Akt has dual profibrotic effects , increasing collagen synthesis and decreasing its degradation via downregulation of MMP1 .
	manualset3
175764	4	413649	7	NULL	NULL	NULL	NULL	dual profibrotic effects	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings suggest that in human dermal fibroblasts , Akt has dual profibrotic effects , increasing collagen synthesis and decreasing its degradation via downregulation of MMP1 .
	manualset3
175765	5	413649	7	NULL	NULL	NULL	NULL	collagen synthesis 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings suggest that in human dermal fibroblasts , Akt has dual profibrotic effects , increasing collagen synthesis and decreasing its degradation via downregulation of MMP1 .
	manualset3
175766	6	413649	7	NULL	NULL	NULL	NULL	degradation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings suggest that in human dermal fibroblasts , Akt has dual profibrotic effects , increasing collagen synthesis and decreasing its degradation via downregulation of MMP1 .
	manualset3
175767	7	413649	7	NULL	NULL	NULL	NULL	downregulation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings suggest that in human dermal fibroblasts , Akt has dual profibrotic effects , increasing collagen synthesis and decreasing its degradation via downregulation of MMP1 .
	manualset3
175768	8	413649	7	NULL	NULL	0	NULL	MMP1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that in human dermal fibroblasts , Akt has dual profibrotic effects , increasing collagen synthesis and decreasing its degradation via downregulation of MMP1 .
	manualset3
175769	1	413650	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that ondansetron does not possess physical dependence liability , but does potentiate the development of physical dependence on diazepam .
	manualset3
175770	2	413650	7	NULL	NULL	0	NULL	 ondansetron	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that ondansetron does not possess physical dependence liability , but does potentiate the development of physical dependence on diazepam .
	manualset3
175771	3	413650	7	NULL	NULL	0	NULL	physical dependence liability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that ondansetron does not possess physical dependence liability , but does potentiate the development of physical dependence on diazepam .
	manualset3
175772	4	413650	7	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that ondansetron does not possess physical dependence liability , but does potentiate the development of physical dependence on diazepam .
	manualset3
175773	5	413650	7	NULL	NULL	0	NULL	physical dependence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that ondansetron does not possess physical dependence liability , but does potentiate the development of physical dependence on diazepam .
	manualset3
175774	6	413650	7	NULL	NULL	0	NULL	diazepam	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that ondansetron does not possess physical dependence liability , but does potentiate the development of physical dependence on diazepam .
	manualset3
175775	1	413651	7	NULL	NULL	0	NULL	 findings 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that organization need to create the policy consistent with community need and provide clear goal and instruction to improve to motivation and performance of CFs .
	manualset3
175776	2	413651	7	NULL	NULL	0	NULL	organization	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that organization need to create the policy consistent with community need and provide clear goal and instruction to improve to motivation and performance of CFs .
	manualset3
175777	3	413651	7	NULL	NULL	0	NULL	policy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that organization need to create the policy consistent with community need and provide clear goal and instruction to improve to motivation and performance of CFs .
	manualset3
175778	4	413651	7	NULL	NULL	0	NULL	community need	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that organization need to create the policy consistent with community need and provide clear goal and instruction to improve to motivation and performance of CFs .
	manualset3
175779	5	413651	7	NULL	NULL	0	NULL	clear goal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that organization need to create the policy consistent with community need and provide clear goal and instruction to improve to motivation and performance of CFs .
	manualset3
175780	6	413651	7	NULL	NULL	0	NULL	instruction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that organization need to create the policy consistent with community need and provide clear goal and instruction to improve to motivation and performance of CFs .
	manualset3
175781	7	413651	7	NULL	NULL	0	NULL	motivation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that organization need to create the policy consistent with community need and provide clear goal and instruction to improve to motivation and performance of CFs .
	manualset3
175782	8	413651	7	NULL	NULL	0	NULL	performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that organization need to create the policy consistent with community need and provide clear goal and instruction to improve to motivation and performance of CFs .
	manualset3
175783	9	413651	7	NULL	NULL	NULL	NULL	CFs	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings suggest that organization need to create the policy consistent with community need and provide clear goal and instruction to improve to motivation and performance of CFs .
	manualset3
175784	1	413652	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that small RNA pathways are activated in the egg cell in both rice and Arabidopsis .
	manualset3
175785	2	413652	7	NULL	NULL	0	NULL	small RNA pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that small RNA pathways are activated in the egg cell in both rice and Arabidopsis .
	manualset3
175786	3	413652	7	NULL	NULL	0	NULL	egg cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that small RNA pathways are activated in the egg cell in both rice and Arabidopsis .
	manualset3
175787	4	413652	7	NULL	NULL	0	NULL	rice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that small RNA pathways are activated in the egg cell in both rice and Arabidopsis .
	manualset3
175788	5	413652	7	NULL	NULL	0	NULL	Arabidopsis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that small RNA pathways are activated in the egg cell in both rice and Arabidopsis .
	manualset3
175789	1	413653	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the Ministry of Health should recommend an interim policy with AQ + SP combination as the first-line antimalarial drug in Bangui until best alternative treatments like artemisinin-based combination therapies ( ACTs ) become available at low prices in the CAR .
	manualset3
175790	2	413653	7	NULL	NULL	0	NULL	Ministry of Health	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the Ministry of Health should recommend an interim policy with AQ + SP combination as the first-line antimalarial drug in Bangui until best alternative treatments like artemisinin-based combination therapies ( ACTs ) become available at low prices in the CAR .
	manualset3
175791	3	413653	7	NULL	NULL	0	NULL	 interim policy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the Ministry of Health should recommend an interim policy with AQ + SP combination as the first-line antimalarial drug in Bangui until best alternative treatments like artemisinin-based combination therapies ( ACTs ) become available at low prices in the CAR .
	manualset3
175792	4	413653	7	NULL	NULL	0	NULL	AQ + SP combination	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the Ministry of Health should recommend an interim policy with AQ + SP combination as the first-line antimalarial drug in Bangui until best alternative treatments like artemisinin-based combination therapies ( ACTs ) become available at low prices in the CAR .
	manualset3
175793	5	413653	7	NULL	NULL	0	NULL	antimalarial drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the Ministry of Health should recommend an interim policy with AQ + SP combination as the first-line antimalarial drug in Bangui until best alternative treatments like artemisinin-based combination therapies ( ACTs ) become available at low prices in the CAR .
	manualset3
175794	6	413653	7	NULL	NULL	0	NULL	Bangui	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the Ministry of Health should recommend an interim policy with AQ + SP combination as the first-line antimalarial drug in Bangui until best alternative treatments like artemisinin-based combination therapies ( ACTs ) become available at low prices in the CAR .
	manualset3
175795	7	413653	7	NULL	NULL	0	NULL	alternative treatments 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the Ministry of Health should recommend an interim policy with AQ + SP combination as the first-line antimalarial drug in Bangui until best alternative treatments like artemisinin-based combination therapies ( ACTs ) become available at low prices in the CAR .
	manualset3
175796	8	413653	7	NULL	NULL	0	NULL	artemisinin-based combination therapies ( ACTs )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the Ministry of Health should recommend an interim policy with AQ + SP combination as the first-line antimalarial drug in Bangui until best alternative treatments like artemisinin-based combination therapies ( ACTs ) become available at low prices in the CAR .
	manualset3
175797	9	413653	7	NULL	NULL	0	NULL	low prices 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the Ministry of Health should recommend an interim policy with AQ + SP combination as the first-line antimalarial drug in Bangui until best alternative treatments like artemisinin-based combination therapies ( ACTs ) become available at low prices in the CAR .
	manualset3
175798	10	413653	7	NULL	NULL	0	NULL	CAR	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the Ministry of Health should recommend an interim policy with AQ + SP combination as the first-line antimalarial drug in Bangui until best alternative treatments like artemisinin-based combination therapies ( ACTs ) become available at low prices in the CAR .
	manualset3
175799	1	413654	7	NULL	NULL	0	NULL	findings 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the beneficial vascular effects of ACE inhibition in heart failure may be due in part to improved endothelial function .
	manualset3
175800	2	413654	7	NULL	NULL	0	NULL	vascular effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the beneficial vascular effects of ACE inhibition in heart failure may be due in part to improved endothelial function .
	manualset3
175801	3	413654	7	NULL	NULL	0	NULL	ACE inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the beneficial vascular effects of ACE inhibition in heart failure may be due in part to improved endothelial function .
	manualset3
175802	4	413654	7	NULL	NULL	0	NULL	 heart failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the beneficial vascular effects of ACE inhibition in heart failure may be due in part to improved endothelial function .
	manualset3
175803	5	413654	7	NULL	NULL	0	NULL	endothelial function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the beneficial vascular effects of ACE inhibition in heart failure may be due in part to improved endothelial function .
	manualset3
175804	1	413655	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the etiology of adult AML can not be explained by polymorphism at a single locus , perhaps because of complexity involved in the metabolism of diverse xenobiotic compounds , and therefore , multiple gene-gene interactions should be investigated to predict the risk of AML .
	manualset3
175805	2	413655	7	NULL	NULL	0	NULL	etiology	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the etiology of adult AML can not be explained by polymorphism at a single locus , perhaps because of complexity involved in the metabolism of diverse xenobiotic compounds , and therefore , multiple gene-gene interactions should be investigated to predict the risk of AML .
	manualset3
175806	3	413655	7	NULL	NULL	0	NULL	adult AML	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the etiology of adult AML can not be explained by polymorphism at a single locus , perhaps because of complexity involved in the metabolism of diverse xenobiotic compounds , and therefore , multiple gene-gene interactions should be investigated to predict the risk of AML .
	manualset3
175807	4	413655	7	NULL	NULL	0	NULL	polymorphism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the etiology of adult AML can not be explained by polymorphism at a single locus , perhaps because of complexity involved in the metabolism of diverse xenobiotic compounds , and therefore , multiple gene-gene interactions should be investigated to predict the risk of AML .
	manualset3
175808	5	413655	7	NULL	NULL	0	NULL	single locus	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the etiology of adult AML can not be explained by polymorphism at a single locus , perhaps because of complexity involved in the metabolism of diverse xenobiotic compounds , and therefore , multiple gene-gene interactions should be investigated to predict the risk of AML .
	manualset3
175809	6	413655	7	NULL	NULL	0	NULL	complexity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the etiology of adult AML can not be explained by polymorphism at a single locus , perhaps because of complexity involved in the metabolism of diverse xenobiotic compounds , and therefore , multiple gene-gene interactions should be investigated to predict the risk of AML .
	manualset3
175810	7	413655	7	NULL	NULL	0	NULL	metabolism 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the etiology of adult AML can not be explained by polymorphism at a single locus , perhaps because of complexity involved in the metabolism of diverse xenobiotic compounds , and therefore , multiple gene-gene interactions should be investigated to predict the risk of AML .
	manualset3
175811	8	413655	7	NULL	NULL	0	NULL	xenobiotic compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the etiology of adult AML can not be explained by polymorphism at a single locus , perhaps because of complexity involved in the metabolism of diverse xenobiotic compounds , and therefore , multiple gene-gene interactions should be investigated to predict the risk of AML .
	manualset3
175812	9	413655	7	NULL	NULL	0	NULL	multiple gene-gene interactions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the etiology of adult AML can not be explained by polymorphism at a single locus , perhaps because of complexity involved in the metabolism of diverse xenobiotic compounds , and therefore , multiple gene-gene interactions should be investigated to predict the risk of AML .
	manualset3
175813	10	413655	7	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the etiology of adult AML can not be explained by polymorphism at a single locus , perhaps because of complexity involved in the metabolism of diverse xenobiotic compounds , and therefore , multiple gene-gene interactions should be investigated to predict the risk of AML .
	manualset3
175814	11	413655	7	NULL	NULL	0	NULL	AML	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the etiology of adult AML can not be explained by polymorphism at a single locus , perhaps because of complexity involved in the metabolism of diverse xenobiotic compounds , and therefore , multiple gene-gene interactions should be investigated to predict the risk of AML .
	manualset3
175815	1	413656	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the functional tone of the 5-HTergic projection to the FPCx is stronger in the RHA/Verh line relative to the RLA/Verh line .
	manualset3
175816	2	413656	7	NULL	NULL	0	NULL	 functional tone	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the functional tone of the 5-HTergic projection to the FPCx is stronger in the RHA/Verh line relative to the RLA/Verh line .
	manualset3
175817	3	413656	7	NULL	NULL	0	NULL	 5-HTergic projection 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the functional tone of the 5-HTergic projection to the FPCx is stronger in the RHA/Verh line relative to the RLA/Verh line .
	manualset3
175818	4	413656	7	NULL	NULL	0	NULL	FPCx 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the functional tone of the 5-HTergic projection to the FPCx is stronger in the RHA/Verh line relative to the RLA/Verh line .
	manualset3
175819	5	413656	7	NULL	NULL	0	NULL	RHA/Verh line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the functional tone of the 5-HTergic projection to the FPCx is stronger in the RHA/Verh line relative to the RLA/Verh line .
	manualset3
175820	6	413656	7	NULL	NULL	0	NULL	RLA/Verh line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the functional tone of the 5-HTergic projection to the FPCx is stronger in the RHA/Verh line relative to the RLA/Verh line .
	manualset3
175821	1	413657	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the medial temporal lobe may be central to the generation of novel ideas and creative evaluation may extend beyond deliberate analytical processes supported by executive brain regions to include more spontaneous affective and visceroceptive evaluative processes supported by default and limbic regions .
	manualset3
175822	2	413657	7	NULL	NULL	0	NULL	medial temporal lobe	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the medial temporal lobe may be central to the generation of novel ideas and creative evaluation may extend beyond deliberate analytical processes supported by executive brain regions to include more spontaneous affective and visceroceptive evaluative processes supported by default and limbic regions .
	manualset3
175823	3	413657	7	NULL	NULL	0	NULL	generation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the medial temporal lobe may be central to the generation of novel ideas and creative evaluation may extend beyond deliberate analytical processes supported by executive brain regions to include more spontaneous affective and visceroceptive evaluative processes supported by default and limbic regions .
	manualset3
175824	4	413657	7	NULL	NULL	0	NULL	novel ideas	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the medial temporal lobe may be central to the generation of novel ideas and creative evaluation may extend beyond deliberate analytical processes supported by executive brain regions to include more spontaneous affective and visceroceptive evaluative processes supported by default and limbic regions .
	manualset3
175825	5	413657	7	NULL	NULL	0	NULL	creative evaluation	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the medial temporal lobe may be central to the generation of novel ideas and creative evaluation may extend beyond deliberate analytical processes supported by executive brain regions to include more spontaneous affective and visceroceptive evaluative processes supported by default and limbic regions .
	manualset3
175826	6	413657	7	NULL	NULL	0	NULL	analytical processes	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the medial temporal lobe may be central to the generation of novel ideas and creative evaluation may extend beyond deliberate analytical processes supported by executive brain regions to include more spontaneous affective and visceroceptive evaluative processes supported by default and limbic regions .
	manualset3
175827	7	413657	7	NULL	NULL	0	NULL	executive brain regions 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the medial temporal lobe may be central to the generation of novel ideas and creative evaluation may extend beyond deliberate analytical processes supported by executive brain regions to include more spontaneous affective and visceroceptive evaluative processes supported by default and limbic regions .
	manualset3
175828	8	413657	7	NULL	NULL	0	NULL	affective evaluative processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the medial temporal lobe may be central to the generation of novel ideas and creative evaluation may extend beyond deliberate analytical processes supported by executive brain regions to include more spontaneous affective and visceroceptive evaluative processes supported by default and limbic regions .
	manualset3
175829	9	413657	7	NULL	NULL	0	NULL	visceroceptive evaluative processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the medial temporal lobe may be central to the generation of novel ideas and creative evaluation may extend beyond deliberate analytical processes supported by executive brain regions to include more spontaneous affective and visceroceptive evaluative processes supported by default and limbic regions .
	manualset3
175830	10	413657	7	NULL	NULL	0	NULL	 limbic regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that the medial temporal lobe may be central to the generation of novel ideas and creative evaluation may extend beyond deliberate analytical processes supported by executive brain regions to include more spontaneous affective and visceroceptive evaluative processes supported by default and limbic regions .
	manualset3
175831	1	413658	7	NULL	NULL	0	NULL	Addition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of SP-B + C further decreased ventilatory pressures to levels similar to LES ( p & lt ; 0.01 versus control , lipid-only surfactants ) .
	manualset3
175832	2	413658	7	NULL	NULL	0	NULL	SP-B + C	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of SP-B + C further decreased ventilatory pressures to levels similar to LES ( p & lt ; 0.01 versus control , lipid-only surfactants ) .
	manualset3
175833	3	413658	7	NULL	NULL	0	NULL	ventilatory pressures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of SP-B + C further decreased ventilatory pressures to levels similar to LES ( p & lt ; 0.01 versus control , lipid-only surfactants ) .
	manualset3
175834	4	413658	7	NULL	NULL	0	NULL	levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of SP-B + C further decreased ventilatory pressures to levels similar to LES ( p & lt ; 0.01 versus control , lipid-only surfactants ) .
	manualset3
175835	5	413658	7	NULL	NULL	0	NULL	 LES 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of SP-B + C further decreased ventilatory pressures to levels similar to LES ( p & lt ; 0.01 versus control , lipid-only surfactants ) .
	manualset3
175836	6	413658	7	NULL	NULL	0	NULL	 p & lt 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of SP-B + C further decreased ventilatory pressures to levels similar to LES ( p & lt ; 0.01 versus control , lipid-only surfactants ) .
	manualset3
175837	7	413658	7	NULL	NULL	0	NULL	control 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of SP-B + C further decreased ventilatory pressures to levels similar to LES ( p & lt ; 0.01 versus control , lipid-only surfactants ) .
	manualset3
175838	8	413658	7	NULL	NULL	0	NULL	lipid-only surfactants	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of SP-B + C further decreased ventilatory pressures to levels similar to LES ( p & lt ; 0.01 versus control , lipid-only surfactants ) .
	manualset3
175839	1	413659	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that there is a difference between the anteromedial frontal cortex and the caudate putamen with respect to the regulating mechanism of dopamine release and its metabolism .
	manualset3
175840	2	413659	7	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that there is a difference between the anteromedial frontal cortex and the caudate putamen with respect to the regulating mechanism of dopamine release and its metabolism .
	manualset3
175841	3	413659	7	NULL	NULL	0	NULL	anteromedial frontal cortex 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that there is a difference between the anteromedial frontal cortex and the caudate putamen with respect to the regulating mechanism of dopamine release and its metabolism .
	manualset3
175842	4	413659	7	NULL	NULL	0	NULL	caudate putamen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that there is a difference between the anteromedial frontal cortex and the caudate putamen with respect to the regulating mechanism of dopamine release and its metabolism .
	manualset3
175843	5	413659	7	NULL	NULL	NULL	NULL	mechanism	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings suggest that there is a difference between the anteromedial frontal cortex and the caudate putamen with respect to the regulating mechanism of dopamine release and its metabolism .
	manualset3
175844	6	413659	7	NULL	NULL	0	NULL	dopamine release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that there is a difference between the anteromedial frontal cortex and the caudate putamen with respect to the regulating mechanism of dopamine release and its metabolism .
	manualset3
175845	7	413659	7	NULL	NULL	0	NULL	metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest that there is a difference between the anteromedial frontal cortex and the caudate putamen with respect to the regulating mechanism of dopamine release and its metabolism .
	manualset3
175846	1	413660	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest the importance of assessing functional limitations in individuals with mood disorders , especially those living in disadvantaged economic conditions .
	manualset3
175847	2	413660	7	NULL	NULL	0	NULL	functional limitations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest the importance of assessing functional limitations in individuals with mood disorders , especially those living in disadvantaged economic conditions .
	manualset3
175848	3	413660	7	NULL	NULL	0	NULL	individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest the importance of assessing functional limitations in individuals with mood disorders , especially those living in disadvantaged economic conditions .
	manualset3
175849	4	413660	7	NULL	NULL	0	NULL	mood disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest the importance of assessing functional limitations in individuals with mood disorders , especially those living in disadvantaged economic conditions .
	manualset3
175850	5	413660	7	NULL	NULL	0	NULL	economic conditions	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest the importance of assessing functional limitations in individuals with mood disorders , especially those living in disadvantaged economic conditions .
	manualset3
175851	6	413660	7	NULL	NULL	0	NULL	 living	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest the importance of assessing functional limitations in individuals with mood disorders , especially those living in disadvantaged economic conditions .
	manualset3
175852	1	413661	7	NULL	NULL	0	NULL	findings 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest thyroid hyperfunction in the molar pregnancy is due to a larger amount of HCT than in normal pregnancy .
	manualset3
175853	2	413661	7	NULL	NULL	0	NULL	thyroid hyperfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest thyroid hyperfunction in the molar pregnancy is due to a larger amount of HCT than in normal pregnancy .
	manualset3
175854	3	413661	7	NULL	NULL	0	NULL	molar pregnancy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest thyroid hyperfunction in the molar pregnancy is due to a larger amount of HCT than in normal pregnancy .
	manualset3
175855	4	413661	7	NULL	NULL	0	NULL	 larger amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest thyroid hyperfunction in the molar pregnancy is due to a larger amount of HCT than in normal pregnancy .
	manualset3
175856	5	413661	7	NULL	NULL	0	NULL	HCT	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest thyroid hyperfunction in the molar pregnancy is due to a larger amount of HCT than in normal pregnancy .
	manualset3
175857	6	413661	7	NULL	NULL	0	NULL	normal pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings suggest thyroid hyperfunction in the molar pregnancy is due to a larger amount of HCT than in normal pregnancy .
	manualset3
175858	1	413662	7	NULL	NULL	0	NULL	 findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings support the hypothesis that the 30 , 000 MW Cd-BP is a plausible target of Cd in Cd-induced testicular injury , and suggest a basis for the peculiar sensitivity of the rat testis to Cd .
	manualset3
175859	2	413662	7	NULL	NULL	0	NULL	hypothesis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings support the hypothesis that the 30 , 000 MW Cd-BP is a plausible target of Cd in Cd-induced testicular injury , and suggest a basis for the peculiar sensitivity of the rat testis to Cd .
	manualset3
175860	3	413662	7	NULL	NULL	0	NULL	30 , 000 MW	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings support the hypothesis that the 30 , 000 MW Cd-BP is a plausible target of Cd in Cd-induced testicular injury , and suggest a basis for the peculiar sensitivity of the rat testis to Cd .
	manualset3
175861	4	413662	7	NULL	NULL	0	NULL	 Cd-BP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings support the hypothesis that the 30 , 000 MW Cd-BP is a plausible target of Cd in Cd-induced testicular injury , and suggest a basis for the peculiar sensitivity of the rat testis to Cd .
	manualset3
175862	5	413662	7	NULL	NULL	0	NULL	plausible target	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings support the hypothesis that the 30 , 000 MW Cd-BP is a plausible target of Cd in Cd-induced testicular injury , and suggest a basis for the peculiar sensitivity of the rat testis to Cd .
	manualset3
175863	6	413662	7	NULL	NULL	0	NULL	Cd	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings support the hypothesis that the 30 , 000 MW Cd-BP is a plausible target of Cd in Cd-induced testicular injury , and suggest a basis for the peculiar sensitivity of the rat testis to Cd .
	manualset3
175864	7	413662	7	NULL	NULL	0	NULL	Cd-induced testicular injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings support the hypothesis that the 30 , 000 MW Cd-BP is a plausible target of Cd in Cd-induced testicular injury , and suggest a basis for the peculiar sensitivity of the rat testis to Cd .
	manualset3
175865	8	413662	7	NULL	NULL	0	NULL	peculiar sensitivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings support the hypothesis that the 30 , 000 MW Cd-BP is a plausible target of Cd in Cd-induced testicular injury , and suggest a basis for the peculiar sensitivity of the rat testis to Cd .
	manualset3
175866	9	413662	7	NULL	NULL	0	NULL	 rat testis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings support the hypothesis that the 30 , 000 MW Cd-BP is a plausible target of Cd in Cd-induced testicular injury , and suggest a basis for the peculiar sensitivity of the rat testis to Cd .
	manualset3
175867	10	413662	7	NULL	NULL	0	NULL	Cd	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings support the hypothesis that the 30 , 000 MW Cd-BP is a plausible target of Cd in Cd-induced testicular injury , and suggest a basis for the peculiar sensitivity of the rat testis to Cd .
	manualset3
175868	1	413663	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings support the notion that FQ could be useful in treating persons with P. falciparum malaria .
	manualset3
175869	2	413663	7	NULL	NULL	0	NULL	notion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings support the notion that FQ could be useful in treating persons with P. falciparum malaria .
	manualset3
175870	3	413663	7	NULL	NULL	0	NULL	FQ	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings support the notion that FQ could be useful in treating persons with P. falciparum malaria .
	manualset3
175871	4	413663	7	NULL	NULL	0	NULL	persons	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings support the notion that FQ could be useful in treating persons with P. falciparum malaria .
	manualset3
175872	5	413663	7	NULL	NULL	0	NULL	P. falciparum malaria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings support the notion that FQ could be useful in treating persons with P. falciparum malaria .
	manualset3
175874	1	413664	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings were further confirmed by histopathological study of liver .
	manualset3
175875	2	413664	7	NULL	NULL	0	NULL	histopathological study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings were further confirmed by histopathological study of liver .
	manualset3
175876	3	413664	7	NULL	NULL	0	NULL	 liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings were further confirmed by histopathological study of liver .
	manualset3
175877	1	413665	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings were in concert with an efficiency model of neurolinguistic organization that suggests that the left hemisphere is dominant for language processing with the right hemisphere being capable of performing less efficient auditory-verbal analysis .
	manualset3
175878	2	413665	7	NULL	NULL	0	NULL	 efficiency model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings were in concert with an efficiency model of neurolinguistic organization that suggests that the left hemisphere is dominant for language processing with the right hemisphere being capable of performing less efficient auditory-verbal analysis .
	manualset3
175879	3	413665	7	NULL	NULL	0	NULL	 neurolinguistic organization	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings were in concert with an efficiency model of neurolinguistic organization that suggests that the left hemisphere is dominant for language processing with the right hemisphere being capable of performing less efficient auditory-verbal analysis .
	manualset3
175880	4	413665	7	NULL	NULL	0	NULL	left hemisphere 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings were in concert with an efficiency model of neurolinguistic organization that suggests that the left hemisphere is dominant for language processing with the right hemisphere being capable of performing less efficient auditory-verbal analysis .
	manualset3
175881	5	413665	7	NULL	NULL	0	NULL	language processing	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings were in concert with an efficiency model of neurolinguistic organization that suggests that the left hemisphere is dominant for language processing with the right hemisphere being capable of performing less efficient auditory-verbal analysis .
	manualset3
175882	6	413665	7	NULL	NULL	0	NULL	 right hemisphere 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings were in concert with an efficiency model of neurolinguistic organization that suggests that the left hemisphere is dominant for language processing with the right hemisphere being capable of performing less efficient auditory-verbal analysis .
	manualset3
175884	8	413665	7	NULL	NULL	NULL	NULL	auditory-verbal analysis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These findings were in concert with an efficiency model of neurolinguistic organization that suggests that the left hemisphere is dominant for language processing with the right hemisphere being capable of performing less efficient auditory-verbal analysis .
	manualset3
175885	1	413666	7	NULL	NULL	0	NULL	Addition 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of coronatin-1 into primary in vitro cultures of G. mellonella hemocytes resulted in rapid disintegration of spherulocytes freely floating in culture medium and shrinkage of plasmatocytes adhering to the bottom of culture well .
	manualset3
175886	2	413666	7	NULL	NULL	0	NULL	coronatin-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of coronatin-1 into primary in vitro cultures of G. mellonella hemocytes resulted in rapid disintegration of spherulocytes freely floating in culture medium and shrinkage of plasmatocytes adhering to the bottom of culture well .
	manualset3
175887	3	413666	7	NULL	NULL	0	NULL	primary in vitro cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of coronatin-1 into primary in vitro cultures of G. mellonella hemocytes resulted in rapid disintegration of spherulocytes freely floating in culture medium and shrinkage of plasmatocytes adhering to the bottom of culture well .
	manualset3
175888	4	413666	7	NULL	NULL	0	NULL	G. mellonella hemocytes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of coronatin-1 into primary in vitro cultures of G. mellonella hemocytes resulted in rapid disintegration of spherulocytes freely floating in culture medium and shrinkage of plasmatocytes adhering to the bottom of culture well .
	manualset3
175889	5	413666	7	NULL	NULL	0	NULL	rapid disintegration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of coronatin-1 into primary in vitro cultures of G. mellonella hemocytes resulted in rapid disintegration of spherulocytes freely floating in culture medium and shrinkage of plasmatocytes adhering to the bottom of culture well .
	manualset3
175890	6	413666	7	NULL	NULL	0	NULL	spherulocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of coronatin-1 into primary in vitro cultures of G. mellonella hemocytes resulted in rapid disintegration of spherulocytes freely floating in culture medium and shrinkage of plasmatocytes adhering to the bottom of culture well .
	manualset3
175891	7	413666	7	NULL	NULL	0	NULL	culture medium	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of coronatin-1 into primary in vitro cultures of G. mellonella hemocytes resulted in rapid disintegration of spherulocytes freely floating in culture medium and shrinkage of plasmatocytes adhering to the bottom of culture well .
	manualset3
175892	8	413666	7	NULL	NULL	0	NULL	shrinkage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of coronatin-1 into primary in vitro cultures of G. mellonella hemocytes resulted in rapid disintegration of spherulocytes freely floating in culture medium and shrinkage of plasmatocytes adhering to the bottom of culture well .
	manualset3
175893	9	413666	7	NULL	NULL	0	NULL	plasmatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of coronatin-1 into primary in vitro cultures of G. mellonella hemocytes resulted in rapid disintegration of spherulocytes freely floating in culture medium and shrinkage of plasmatocytes adhering to the bottom of culture well .
	manualset3
175894	10	413666	7	NULL	NULL	0	NULL	bottom 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of coronatin-1 into primary in vitro cultures of G. mellonella hemocytes resulted in rapid disintegration of spherulocytes freely floating in culture medium and shrinkage of plasmatocytes adhering to the bottom of culture well .
	manualset3
175895	11	413666	7	NULL	NULL	0	NULL	culture well	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of coronatin-1 into primary in vitro cultures of G. mellonella hemocytes resulted in rapid disintegration of spherulocytes freely floating in culture medium and shrinkage of plasmatocytes adhering to the bottom of culture well .
	manualset3
175896	1	413667	7	NULL	NULL	0	NULL	 four subgroups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These four subgroups differed significantly on a number of sociodemographic , health status and health service use characteristics but no significant differences were found in satisfaction between preference segments .
	manualset3
175897	2	413667	7	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These four subgroups differed significantly on a number of sociodemographic , health status and health service use characteristics but no significant differences were found in satisfaction between preference segments .
	manualset3
175898	3	413667	7	NULL	NULL	0	NULL	sociodemographic status	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These four subgroups differed significantly on a number of sociodemographic , health status and health service use characteristics but no significant differences were found in satisfaction between preference segments .
	manualset3
175899	4	413667	7	NULL	NULL	0	NULL	health status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These four subgroups differed significantly on a number of sociodemographic , health status and health service use characteristics but no significant differences were found in satisfaction between preference segments .
	manualset3
175900	5	413667	7	NULL	NULL	0	NULL	health service	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	These four subgroups differed significantly on a number of sociodemographic , health status and health service use characteristics but no significant differences were found in satisfaction between preference segments .
	manualset3
175901	6	413667	7	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These four subgroups differed significantly on a number of sociodemographic , health status and health service use characteristics but no significant differences were found in satisfaction between preference segments .
	manualset3
175902	7	413667	7	NULL	NULL	0	NULL	satisfaction 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These four subgroups differed significantly on a number of sociodemographic , health status and health service use characteristics but no significant differences were found in satisfaction between preference segments .
	manualset3
175903	8	413667	7	NULL	NULL	0	NULL	preference segments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These four subgroups differed significantly on a number of sociodemographic , health status and health service use characteristics but no significant differences were found in satisfaction between preference segments .
	manualset3
190510	9	413667	7	NULL	NULL	0	NULL	 characteristics	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These four subgroups differed significantly on a number of sociodemographic , health status and health service use characteristics but no significant differences were found in satisfaction between preference segments .
	manualset3
175904	1	413668	7	NULL	NULL	0	NULL	 functional roles 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These functional roles may either come from systemic chronic inflammatory or directly signaling pathway within bone cells .
	manualset3
175905	2	413668	7	NULL	NULL	0	NULL	systemic chronic inflammatory pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These functional roles may either come from systemic chronic inflammatory or directly signaling pathway within bone cells .
	manualset3
175906	3	413668	7	NULL	NULL	0	NULL	signaling pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These functional roles may either come from systemic chronic inflammatory or directly signaling pathway within bone cells .
	manualset3
175907	4	413668	7	NULL	NULL	0	NULL	bone cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These functional roles may either come from systemic chronic inflammatory or directly signaling pathway within bone cells .
	manualset3
175969	1	413669	7	NULL	NULL	0	NULL	gene-encoded peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	These gene-encoded peptides have direct antibiotic activity against a wide range of bacteria and other microbes .
	manualset3
175970	2	413669	7	NULL	NULL	0	NULL	antibiotic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These gene-encoded peptides have direct antibiotic activity against a wide range of bacteria and other microbes .
	manualset3
175971	3	413669	7	NULL	NULL	0	NULL	wide range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These gene-encoded peptides have direct antibiotic activity against a wide range of bacteria and other microbes .
	manualset3
175972	4	413669	7	NULL	NULL	0	NULL	 bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These gene-encoded peptides have direct antibiotic activity against a wide range of bacteria and other microbes .
	manualset3
175973	5	413669	7	NULL	NULL	0	NULL	microbes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These gene-encoded peptides have direct antibiotic activity against a wide range of bacteria and other microbes .
	manualset3
175974	1	413670	7	NULL	NULL	0	NULL	 genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These genes code for sarcomeric proteins and exhibit the same phenotype , suggesting that HCM is a disease of the sarcomere .
	manualset3
175975	2	413670	7	NULL	NULL	0	NULL	sarcomeric proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These genes code for sarcomeric proteins and exhibit the same phenotype , suggesting that HCM is a disease of the sarcomere .
	manualset3
175976	3	413670	7	NULL	NULL	0	NULL	phenotype	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These genes code for sarcomeric proteins and exhibit the same phenotype , suggesting that HCM is a disease of the sarcomere .
	manualset3
175977	4	413670	7	NULL	NULL	0	NULL	HCM	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These genes code for sarcomeric proteins and exhibit the same phenotype , suggesting that HCM is a disease of the sarcomere .
	manualset3
175978	5	413670	7	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These genes code for sarcomeric proteins and exhibit the same phenotype , suggesting that HCM is a disease of the sarcomere .
	manualset3
175979	6	413670	7	NULL	NULL	0	NULL	sarcomere	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These genes code for sarcomeric proteins and exhibit the same phenotype , suggesting that HCM is a disease of the sarcomere .
	manualset3
175980	1	413671	7	NULL	NULL	0	NULL	glycoproteins 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These glycoproteins possessed the ability to bind hyaluronate .
	manualset3
175981	2	413671	7	NULL	NULL	0	NULL	ability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These glycoproteins possessed the ability to bind hyaluronate .
	manualset3
175982	3	413671	7	NULL	NULL	0	NULL	hyaluronate	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These glycoproteins possessed the ability to bind hyaluronate .
	manualset3
175983	1	413672	7	NULL	NULL	0	NULL	Addition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of fibronectin to fluorescein-labeled collagen chains caused a dose-dependent increase in the fluorescence anisotropy which continued over several logs of titrant concentration .
	manualset3
175984	2	413672	7	NULL	NULL	0	NULL	fibronectin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of fibronectin to fluorescein-labeled collagen chains caused a dose-dependent increase in the fluorescence anisotropy which continued over several logs of titrant concentration .
	manualset3
175985	3	413672	7	NULL	NULL	0	NULL	fluorescein-labeled collagen chains	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of fibronectin to fluorescein-labeled collagen chains caused a dose-dependent increase in the fluorescence anisotropy which continued over several logs of titrant concentration .
	manualset3
175986	4	413672	7	NULL	NULL	0	NULL	dose-dependent increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of fibronectin to fluorescein-labeled collagen chains caused a dose-dependent increase in the fluorescence anisotropy which continued over several logs of titrant concentration .
	manualset3
175987	5	413672	7	NULL	NULL	0	NULL	fluorescence anisotropy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of fibronectin to fluorescein-labeled collagen chains caused a dose-dependent increase in the fluorescence anisotropy which continued over several logs of titrant concentration .
	manualset3
175988	6	413672	7	NULL	NULL	0	NULL	several logs	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of fibronectin to fluorescein-labeled collagen chains caused a dose-dependent increase in the fluorescence anisotropy which continued over several logs of titrant concentration .
	manualset3
175989	7	413672	7	NULL	NULL	0	NULL	 titrant concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of fibronectin to fluorescein-labeled collagen chains caused a dose-dependent increase in the fluorescence anisotropy which continued over several logs of titrant concentration .
	manualset3
175990	1	413673	7	NULL	NULL	0	NULL	guidelines	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These guidelines serve as selection criteria to help determine not only which members of the insured population receive treatment for mental health care , but also to determine the allocation of enrollees to staff members and to prescribe the starting point for the types of services received .
	manualset3
175992	2	413673	7	NULL	NULL	0	NULL	members	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These guidelines serve as selection criteria to help determine not only which members of the insured population receive treatment for mental health care , but also to determine the allocation of enrollees to staff members and to prescribe the starting point for the types of services received .
	manualset3
175993	3	413673	7	NULL	NULL	0	NULL	insured population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These guidelines serve as selection criteria to help determine not only which members of the insured population receive treatment for mental health care , but also to determine the allocation of enrollees to staff members and to prescribe the starting point for the types of services received .
	manualset3
175995	4	413673	7	NULL	NULL	0	NULL	 treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These guidelines serve as selection criteria to help determine not only which members of the insured population receive treatment for mental health care , but also to determine the allocation of enrollees to staff members and to prescribe the starting point for the types of services received .
	manualset3
175996	5	413673	7	NULL	NULL	0	NULL	mental health care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These guidelines serve as selection criteria to help determine not only which members of the insured population receive treatment for mental health care , but also to determine the allocation of enrollees to staff members and to prescribe the starting point for the types of services received .
	manualset3
175998	6	413673	7	NULL	NULL	0	NULL	allocation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These guidelines serve as selection criteria to help determine not only which members of the insured population receive treatment for mental health care , but also to determine the allocation of enrollees to staff members and to prescribe the starting point for the types of services received .
	manualset3
175999	7	413673	7	NULL	NULL	0	NULL	enrollees	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These guidelines serve as selection criteria to help determine not only which members of the insured population receive treatment for mental health care , but also to determine the allocation of enrollees to staff members and to prescribe the starting point for the types of services received .
	manualset3
176000	8	413673	7	NULL	NULL	0	NULL	staff members	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These guidelines serve as selection criteria to help determine not only which members of the insured population receive treatment for mental health care , but also to determine the allocation of enrollees to staff members and to prescribe the starting point for the types of services received .
	manualset3
176001	9	413673	7	NULL	NULL	0	NULL	starting point 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These guidelines serve as selection criteria to help determine not only which members of the insured population receive treatment for mental health care , but also to determine the allocation of enrollees to staff members and to prescribe the starting point for the types of services received .
	manualset3
176002	10	413673	7	NULL	NULL	NULL	NULL	types 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These guidelines serve as selection criteria to help determine not only which members of the insured population receive treatment for mental health care , but also to determine the allocation of enrollees to staff members and to prescribe the starting point for the types of services received .
	manualset3
176003	11	413673	7	NULL	NULL	0	NULL	services	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These guidelines serve as selection criteria to help determine not only which members of the insured population receive treatment for mental health care , but also to determine the allocation of enrollees to staff members and to prescribe the starting point for the types of services received .
	manualset3
178199	12	413673	7	NULL	NULL	0	NULL	selection criteria	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These guidelines serve as selection criteria to help determine not only which members of the insured population receive treatment for mental health care , but also to determine the allocation of enrollees to staff members and to prescribe the starting point for the types of services received .
	manualset3
176004	1	413674	7	NULL	NULL	0	NULL	DNA probes XJ1 .1	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These have been tested systematically with the DNA probes XJ1 .1 and pERT87-15 .
	manualset3
176005	2	413674	7	NULL	NULL	0	NULL	 pERT87-15	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These have been tested systematically with the DNA probes XJ1 .1 and pERT87-15 .
	manualset3
176006	1	413675	7	NULL	NULL	0	NULL	 heteroduplexes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These heteroduplexes possessed two types of loops formed as a result of : a ) deletion in one of the DNA strands ; and b ) substitution of a DNA fragment for nonhomological one .
	manualset3
176007	2	413675	7	NULL	NULL	0	NULL	two types	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These heteroduplexes possessed two types of loops formed as a result of : a ) deletion in one of the DNA strands ; and b ) substitution of a DNA fragment for nonhomological one .
	manualset3
176008	3	413675	7	NULL	NULL	NULL	NULL	loops	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These heteroduplexes possessed two types of loops formed as a result of : a ) deletion in one of the DNA strands ; and b ) substitution of a DNA fragment for nonhomological one .
	manualset3
176009	4	413675	7	NULL	NULL	0	NULL	deletion 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These heteroduplexes possessed two types of loops formed as a result of : a ) deletion in one of the DNA strands ; and b ) substitution of a DNA fragment for nonhomological one .
	manualset3
176010	5	413675	7	NULL	NULL	0	NULL	DNA strands	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These heteroduplexes possessed two types of loops formed as a result of : a ) deletion in one of the DNA strands ; and b ) substitution of a DNA fragment for nonhomological one .
	manualset3
176011	6	413675	7	NULL	NULL	NULL	NULL	substitution	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These heteroduplexes possessed two types of loops formed as a result of : a ) deletion in one of the DNA strands ; and b ) substitution of a DNA fragment for nonhomological one .
	manualset3
176012	7	413675	7	NULL	NULL	0	NULL	DNA fragment	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These heteroduplexes possessed two types of loops formed as a result of : a ) deletion in one of the DNA strands ; and b ) substitution of a DNA fragment for nonhomological one .
	manualset3
176022	8	413675	7	NULL	NULL	0	NULL	result	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These heteroduplexes possessed two types of loops formed as a result of : a ) deletion in one of the DNA strands ; and b ) substitution of a DNA fragment for nonhomological one .
	manualset3
190511	9	413675	7	NULL	NULL	0	NULL	 one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These heteroduplexes possessed two types of loops formed as a result of : a ) deletion in one of the DNA strands ; and b ) substitution of a DNA fragment for nonhomological one .
	manualset3
190512	10	413675	7	NULL	NULL	0	NULL	nonhomological one	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These heteroduplexes possessed two types of loops formed as a result of : a ) deletion in one of the DNA strands ; and b ) substitution of a DNA fragment for nonhomological one .
	manualset3
176031	1	413676	7	NULL	NULL	NULL	NULL	high training loads	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These high training loads combined with increasing age could , in part , explain an incidence of non-contact match injuries ( 18 injuries per 1000 match hours ) similar to players , with lower leg muscle strains being the most common type of non-contact injuries in referees .
	manualset3
176032	2	413676	7	NULL	NULL	NULL	NULL	increasing age	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These high training loads combined with increasing age could , in part , explain an incidence of non-contact match injuries ( 18 injuries per 1000 match hours ) similar to players , with lower leg muscle strains being the most common type of non-contact injuries in referees .
	manualset3
176033	3	413676	7	NULL	NULL	0	NULL	non-contact match injuries	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These high training loads combined with increasing age could , in part , explain an incidence of non-contact match injuries ( 18 injuries per 1000 match hours ) similar to players , with lower leg muscle strains being the most common type of non-contact injuries in referees .
	manualset3
176034	4	413676	7	NULL	NULL	0	NULL	18 injuries per 1000 match hours	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These high training loads combined with increasing age could , in part , explain an incidence of non-contact match injuries ( 18 injuries per 1000 match hours ) similar to players , with lower leg muscle strains being the most common type of non-contact injuries in referees .
	manualset3
176035	5	413676	7	NULL	NULL	0	NULL	players	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These high training loads combined with increasing age could , in part , explain an incidence of non-contact match injuries ( 18 injuries per 1000 match hours ) similar to players , with lower leg muscle strains being the most common type of non-contact injuries in referees .
	manualset3
176036	6	413676	7	NULL	NULL	0	NULL	lower leg muscle strains	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These high training loads combined with increasing age could , in part , explain an incidence of non-contact match injuries ( 18 injuries per 1000 match hours ) similar to players , with lower leg muscle strains being the most common type of non-contact injuries in referees .
	manualset3
176037	7	413676	7	NULL	NULL	NULL	NULL	common type	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These high training loads combined with increasing age could , in part , explain an incidence of non-contact match injuries ( 18 injuries per 1000 match hours ) similar to players , with lower leg muscle strains being the most common type of non-contact injuries in referees .
	manualset3
176038	8	413676	7	NULL	NULL	0	NULL	non-contact injuries 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These high training loads combined with increasing age could , in part , explain an incidence of non-contact match injuries ( 18 injuries per 1000 match hours ) similar to players , with lower leg muscle strains being the most common type of non-contact injuries in referees .
	manualset3
176039	9	413676	7	NULL	NULL	0	NULL	referees	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These high training loads combined with increasing age could , in part , explain an incidence of non-contact match injuries ( 18 injuries per 1000 match hours ) similar to players , with lower leg muscle strains being the most common type of non-contact injuries in referees .
	manualset3
176050	1	413677	7	NULL	NULL	0	NULL	phosphorylated proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These highly phosphorylated proteins are secreted at the mineralization front , where a small portion binds in the gap region of type I collagen fibrils .
	manualset3
176051	2	413677	7	NULL	NULL	0	NULL	mineralization front	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These highly phosphorylated proteins are secreted at the mineralization front , where a small portion binds in the gap region of type I collagen fibrils .
	manualset3
176052	3	413677	7	NULL	NULL	0	NULL	small portion	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These highly phosphorylated proteins are secreted at the mineralization front , where a small portion binds in the gap region of type I collagen fibrils .
	manualset3
176053	4	413677	7	NULL	NULL	0	NULL	gap region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These highly phosphorylated proteins are secreted at the mineralization front , where a small portion binds in the gap region of type I collagen fibrils .
	manualset3
176054	5	413677	7	NULL	NULL	0	NULL	 type I collagen fibrils	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These highly phosphorylated proteins are secreted at the mineralization front , where a small portion binds in the gap region of type I collagen fibrils .
	manualset3
176055	1	413678	7	NULL	NULL	0	NULL	progressive tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These highly progressive tumors must represent a very distinct clinical and biological neoplastic entity .
	manualset3
176056	2	413678	7	NULL	NULL	0	NULL	clinical neoplastic entity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These highly progressive tumors must represent a very distinct clinical and biological neoplastic entity .
	manualset3
176057	3	413678	7	NULL	NULL	0	NULL	biological neoplastic entity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These highly progressive tumors must represent a very distinct clinical and biological neoplastic entity .
	manualset3
176079	1	413679	7	NULL	NULL	0	NULL	hinge points 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These hinge points closely correspond to the external limits of wall motion abnormalities .
	manualset3
176080	2	413679	7	NULL	NULL	0	NULL	external limits 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These hinge points closely correspond to the external limits of wall motion abnormalities .
	manualset3
176081	3	413679	7	NULL	NULL	0	NULL	wall motion abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These hinge points closely correspond to the external limits of wall motion abnormalities .
	manualset3
176082	1	413680	7	NULL	NULL	0	NULL	historical control data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These historical control data would help to interpret the effects of test substances in routine toxicity and efficacy studies .
	manualset3
176083	2	413680	7	NULL	NULL	0	NULL	 effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These historical control data would help to interpret the effects of test substances in routine toxicity and efficacy studies .
	manualset3
176085	3	413680	7	NULL	NULL	0	NULL	test substances	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These historical control data would help to interpret the effects of test substances in routine toxicity and efficacy studies .
	manualset3
176088	4	413680	7	NULL	NULL	0	NULL	toxicity studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These historical control data would help to interpret the effects of test substances in routine toxicity and efficacy studies .
	manualset3
176100	5	413680	7	NULL	NULL	0	NULL	efficacy studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These historical control data would help to interpret the effects of test substances in routine toxicity and efficacy studies .
	manualset3
176164	1	413681	7	NULL	NULL	0	NULL	Addition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of gemcitabine to standard therapy in locally advanced cervical cancer : A randomized comparative study .
	manualset3
176165	2	413681	7	NULL	NULL	0	NULL	gemcitabine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of gemcitabine to standard therapy in locally advanced cervical cancer : A randomized comparative study .
	manualset3
176167	3	413681	7	NULL	NULL	0	NULL	standard therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of gemcitabine to standard therapy in locally advanced cervical cancer : A randomized comparative study .
	manualset3
176168	4	413681	7	NULL	NULL	0	NULL	cervical cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of gemcitabine to standard therapy in locally advanced cervical cancer : A randomized comparative study .
	manualset3
176170	5	413681	7	NULL	NULL	0	NULL	comparative study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of gemcitabine to standard therapy in locally advanced cervical cancer : A randomized comparative study .
	manualset3
176173	1	413682	7	NULL	NULL	0	NULL	HSPG	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These include HSPG , Le-y and the H-type-1 antigen , HB-EGF , trophinin-tastin-bystin complex , integrins , and extracellular matrix molecules such as osteopontin and laminin .
	manualset3
176174	2	413682	7	NULL	NULL	0	NULL	Le-y antigen	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These include HSPG , Le-y and the H-type-1 antigen , HB-EGF , trophinin-tastin-bystin complex , integrins , and extracellular matrix molecules such as osteopontin and laminin .
	manualset3
176176	3	413682	7	NULL	NULL	0	NULL	H-type-1 antigen	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These include HSPG , Le-y and the H-type-1 antigen , HB-EGF , trophinin-tastin-bystin complex , integrins , and extracellular matrix molecules such as osteopontin and laminin .
	manualset3
176180	4	413682	7	NULL	NULL	0	NULL	HB-EGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These include HSPG , Le-y and the H-type-1 antigen , HB-EGF , trophinin-tastin-bystin complex , integrins , and extracellular matrix molecules such as osteopontin and laminin .
	manualset3
176181	5	413682	7	NULL	NULL	NULL	NULL	 trophinin-tastin-bystin complex	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These include HSPG , Le-y and the H-type-1 antigen , HB-EGF , trophinin-tastin-bystin complex , integrins , and extracellular matrix molecules such as osteopontin and laminin .
	manualset3
176183	6	413682	7	NULL	NULL	0	NULL	integrins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These include HSPG , Le-y and the H-type-1 antigen , HB-EGF , trophinin-tastin-bystin complex , integrins , and extracellular matrix molecules such as osteopontin and laminin .
	manualset3
176184	7	413682	7	NULL	NULL	0	NULL	extracellular matrix molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	These include HSPG , Le-y and the H-type-1 antigen , HB-EGF , trophinin-tastin-bystin complex , integrins , and extracellular matrix molecules such as osteopontin and laminin .
	manualset3
176185	8	413682	7	NULL	NULL	0	NULL	osteopontin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These include HSPG , Le-y and the H-type-1 antigen , HB-EGF , trophinin-tastin-bystin complex , integrins , and extracellular matrix molecules such as osteopontin and laminin .
	manualset3
176186	9	413682	7	NULL	NULL	0	NULL	laminin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These include HSPG , Le-y and the H-type-1 antigen , HB-EGF , trophinin-tastin-bystin complex , integrins , and extracellular matrix molecules such as osteopontin and laminin .
	manualset3
176190	1	413683	7	NULL	NULL	0	NULL	 acquisition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These include acquisition and transmission of genital HSV-1 and HSV-2 infection , the natural history of genital herpes , and the role of partner notification .
	manualset3
176192	2	413683	7	NULL	NULL	0	NULL	transmission	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These include acquisition and transmission of genital HSV-1 and HSV-2 infection , the natural history of genital herpes , and the role of partner notification .
	manualset3
176193	3	413683	7	NULL	NULL	0	NULL	genital HSV-1 infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These include acquisition and transmission of genital HSV-1 and HSV-2 infection , the natural history of genital herpes , and the role of partner notification .
	manualset3
176194	4	413683	7	NULL	NULL	0	NULL	HSV-2 infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These include acquisition and transmission of genital HSV-1 and HSV-2 infection , the natural history of genital herpes , and the role of partner notification .
	manualset3
176195	5	413683	7	NULL	NULL	0	NULL	natural history	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These include acquisition and transmission of genital HSV-1 and HSV-2 infection , the natural history of genital herpes , and the role of partner notification .
	manualset3
176196	6	413683	7	NULL	NULL	0	NULL	genital herpes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These include acquisition and transmission of genital HSV-1 and HSV-2 infection , the natural history of genital herpes , and the role of partner notification .
	manualset3
176198	7	413683	7	NULL	NULL	NULL	NULL	 role	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These include acquisition and transmission of genital HSV-1 and HSV-2 infection , the natural history of genital herpes , and the role of partner notification .
	manualset3
176200	8	413683	7	NULL	NULL	NULL	NULL	partner notification	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These include acquisition and transmission of genital HSV-1 and HSV-2 infection , the natural history of genital herpes , and the role of partner notification .
	manualset3
176201	1	413684	7	NULL	NULL	0	NULL	fatty acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These include fatty acids of whole cells , of lipopolysaccharides and of single colonies , together with sugar contents of whole cells , of whole defatted cells , of lipopolysaccharides and of single colonies .
	manualset3
176202	2	413684	7	NULL	NULL	0	NULL	whole cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These include fatty acids of whole cells , of lipopolysaccharides and of single colonies , together with sugar contents of whole cells , of whole defatted cells , of lipopolysaccharides and of single colonies .
	manualset3
176203	3	413684	7	NULL	NULL	0	NULL	 lipopolysaccharides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These include fatty acids of whole cells , of lipopolysaccharides and of single colonies , together with sugar contents of whole cells , of whole defatted cells , of lipopolysaccharides and of single colonies .
	manualset3
176204	4	413684	7	NULL	NULL	0	NULL	single colonies	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These include fatty acids of whole cells , of lipopolysaccharides and of single colonies , together with sugar contents of whole cells , of whole defatted cells , of lipopolysaccharides and of single colonies .
	manualset3
176206	5	413684	7	NULL	NULL	0	NULL	sugar contents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These include fatty acids of whole cells , of lipopolysaccharides and of single colonies , together with sugar contents of whole cells , of whole defatted cells , of lipopolysaccharides and of single colonies .
	manualset3
176208	6	413684	7	NULL	NULL	0	NULL	whole cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These include fatty acids of whole cells , of lipopolysaccharides and of single colonies , together with sugar contents of whole cells , of whole defatted cells , of lipopolysaccharides and of single colonies .
	manualset3
176209	7	413684	7	NULL	NULL	0	NULL	whole defatted cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These include fatty acids of whole cells , of lipopolysaccharides and of single colonies , together with sugar contents of whole cells , of whole defatted cells , of lipopolysaccharides and of single colonies .
	manualset3
176212	8	413684	7	NULL	NULL	0	NULL	lipopolysaccharides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These include fatty acids of whole cells , of lipopolysaccharides and of single colonies , together with sugar contents of whole cells , of whole defatted cells , of lipopolysaccharides and of single colonies .
	manualset3
176213	9	413684	7	NULL	NULL	0	NULL	single colonies	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These include fatty acids of whole cells , of lipopolysaccharides and of single colonies , together with sugar contents of whole cells , of whole defatted cells , of lipopolysaccharides and of single colonies .
	manualset3
176218	1	413685	7	NULL	NULL	0	NULL	 improvement 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These include improvement of insulin sensitivity or promotion of insulin resistance , regulation of inflammatory pathways , regulation of glucose transport and tissue glucose uptake , aggravation or attenuation of postprandial glycaemia/insulinaemia , interactions with hormonal responses and - cell-dependent mechanisms .
	manualset3
176219	2	413685	7	NULL	NULL	0	NULL	insulin sensitivity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These include improvement of insulin sensitivity or promotion of insulin resistance , regulation of inflammatory pathways , regulation of glucose transport and tissue glucose uptake , aggravation or attenuation of postprandial glycaemia/insulinaemia , interactions with hormonal responses and - cell-dependent mechanisms .
	manualset3
176220	3	413685	7	NULL	NULL	0	NULL	promotion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These include improvement of insulin sensitivity or promotion of insulin resistance , regulation of inflammatory pathways , regulation of glucose transport and tissue glucose uptake , aggravation or attenuation of postprandial glycaemia/insulinaemia , interactions with hormonal responses and - cell-dependent mechanisms .
	manualset3
176221	4	413685	7	NULL	NULL	0	NULL	insulin resistance	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These include improvement of insulin sensitivity or promotion of insulin resistance , regulation of inflammatory pathways , regulation of glucose transport and tissue glucose uptake , aggravation or attenuation of postprandial glycaemia/insulinaemia , interactions with hormonal responses and - cell-dependent mechanisms .
	manualset3
176222	5	413685	7	NULL	NULL	0	NULL	 regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These include improvement of insulin sensitivity or promotion of insulin resistance , regulation of inflammatory pathways , regulation of glucose transport and tissue glucose uptake , aggravation or attenuation of postprandial glycaemia/insulinaemia , interactions with hormonal responses and - cell-dependent mechanisms .
	manualset3
176223	6	413685	7	NULL	NULL	0	NULL	inflammatory pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These include improvement of insulin sensitivity or promotion of insulin resistance , regulation of inflammatory pathways , regulation of glucose transport and tissue glucose uptake , aggravation or attenuation of postprandial glycaemia/insulinaemia , interactions with hormonal responses and - cell-dependent mechanisms .
	manualset3
176225	7	413685	7	NULL	NULL	0	NULL	 regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These include improvement of insulin sensitivity or promotion of insulin resistance , regulation of inflammatory pathways , regulation of glucose transport and tissue glucose uptake , aggravation or attenuation of postprandial glycaemia/insulinaemia , interactions with hormonal responses and - cell-dependent mechanisms .
	manualset3
176226	8	413685	7	NULL	NULL	0	NULL	glucose transport	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These include improvement of insulin sensitivity or promotion of insulin resistance , regulation of inflammatory pathways , regulation of glucose transport and tissue glucose uptake , aggravation or attenuation of postprandial glycaemia/insulinaemia , interactions with hormonal responses and - cell-dependent mechanisms .
	manualset3
176227	9	413685	7	NULL	NULL	0	NULL	tissue glucose uptake 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These include improvement of insulin sensitivity or promotion of insulin resistance , regulation of inflammatory pathways , regulation of glucose transport and tissue glucose uptake , aggravation or attenuation of postprandial glycaemia/insulinaemia , interactions with hormonal responses and - cell-dependent mechanisms .
	manualset3
176228	10	413685	7	NULL	NULL	0	NULL	aggravation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These include improvement of insulin sensitivity or promotion of insulin resistance , regulation of inflammatory pathways , regulation of glucose transport and tissue glucose uptake , aggravation or attenuation of postprandial glycaemia/insulinaemia , interactions with hormonal responses and - cell-dependent mechanisms .
	manualset3
176230	11	413685	7	NULL	NULL	0	NULL	attenuation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These include improvement of insulin sensitivity or promotion of insulin resistance , regulation of inflammatory pathways , regulation of glucose transport and tissue glucose uptake , aggravation or attenuation of postprandial glycaemia/insulinaemia , interactions with hormonal responses and - cell-dependent mechanisms .
	manualset3
176232	12	413685	7	NULL	NULL	0	NULL	postprandial glycaemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These include improvement of insulin sensitivity or promotion of insulin resistance , regulation of inflammatory pathways , regulation of glucose transport and tissue glucose uptake , aggravation or attenuation of postprandial glycaemia/insulinaemia , interactions with hormonal responses and - cell-dependent mechanisms .
	manualset3
176233	13	413685	7	NULL	NULL	0	NULL	insulinaemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These include improvement of insulin sensitivity or promotion of insulin resistance , regulation of inflammatory pathways , regulation of glucose transport and tissue glucose uptake , aggravation or attenuation of postprandial glycaemia/insulinaemia , interactions with hormonal responses and - cell-dependent mechanisms .
	manualset3
176235	14	413685	7	NULL	NULL	0	NULL	 interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These include improvement of insulin sensitivity or promotion of insulin resistance , regulation of inflammatory pathways , regulation of glucose transport and tissue glucose uptake , aggravation or attenuation of postprandial glycaemia/insulinaemia , interactions with hormonal responses and - cell-dependent mechanisms .
	manualset3
176236	15	413685	7	NULL	NULL	0	NULL	hormonal responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These include improvement of insulin sensitivity or promotion of insulin resistance , regulation of inflammatory pathways , regulation of glucose transport and tissue glucose uptake , aggravation or attenuation of postprandial glycaemia/insulinaemia , interactions with hormonal responses and - cell-dependent mechanisms .
	manualset3
176237	16	413685	7	NULL	NULL	0	NULL	cell-dependent mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These include improvement of insulin sensitivity or promotion of insulin resistance , regulation of inflammatory pathways , regulation of glucose transport and tissue glucose uptake , aggravation or attenuation of postprandial glycaemia/insulinaemia , interactions with hormonal responses and - cell-dependent mechanisms .
	manualset3
176238	1	413686	7	NULL	NULL	0	NULL	pathophysiological mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These include overlapping pathophysiological mechanisms , an unhealthy lifestyle ( poor dietary choices , smoking , lack of exercise ) , genetic factors and a lack of compliance with therapeutic programs .
	manualset3
176239	2	413686	7	NULL	NULL	0	NULL	unhealthy lifestyle	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These include overlapping pathophysiological mechanisms , an unhealthy lifestyle ( poor dietary choices , smoking , lack of exercise ) , genetic factors and a lack of compliance with therapeutic programs .
	manualset3
176240	3	413686	7	NULL	NULL	0	NULL	poor dietary choices	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These include overlapping pathophysiological mechanisms , an unhealthy lifestyle ( poor dietary choices , smoking , lack of exercise ) , genetic factors and a lack of compliance with therapeutic programs .
	manualset3
176241	4	413686	7	NULL	NULL	0	NULL	smoking	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These include overlapping pathophysiological mechanisms , an unhealthy lifestyle ( poor dietary choices , smoking , lack of exercise ) , genetic factors and a lack of compliance with therapeutic programs .
	manualset3
176242	5	413686	7	NULL	NULL	0	NULL	lack of exercise	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These include overlapping pathophysiological mechanisms , an unhealthy lifestyle ( poor dietary choices , smoking , lack of exercise ) , genetic factors and a lack of compliance with therapeutic programs .
	manualset3
176243	6	413686	7	NULL	NULL	0	NULL	genetic factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These include overlapping pathophysiological mechanisms , an unhealthy lifestyle ( poor dietary choices , smoking , lack of exercise ) , genetic factors and a lack of compliance with therapeutic programs .
	manualset3
176245	7	413686	7	NULL	NULL	0	NULL	lack of compliance 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These include overlapping pathophysiological mechanisms , an unhealthy lifestyle ( poor dietary choices , smoking , lack of exercise ) , genetic factors and a lack of compliance with therapeutic programs .
	manualset3
176247	8	413686	7	NULL	NULL	0	NULL	therapeutic programs	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	These include overlapping pathophysiological mechanisms , an unhealthy lifestyle ( poor dietary choices , smoking , lack of exercise ) , genetic factors and a lack of compliance with therapeutic programs .
	manualset3
176249	1	413687	7	NULL	NULL	0	NULL	fibronectin ( alpha 5 beta 1 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These include the well-characterized fibronectin ( alpha 5 beta 1 ) and the multi-specific laminin , collagen and fibronectin ( alpha 3 beta 1 ) receptors .
	manualset3
176257	2	413687	7	NULL	NULL	0	NULL	multi-specific laminin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These include the well-characterized fibronectin ( alpha 5 beta 1 ) and the multi-specific laminin , collagen and fibronectin ( alpha 3 beta 1 ) receptors .
	manualset3
176258	3	413687	7	NULL	NULL	0	NULL	collagen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These include the well-characterized fibronectin ( alpha 5 beta 1 ) and the multi-specific laminin , collagen and fibronectin ( alpha 3 beta 1 ) receptors .
	manualset3
176259	4	413687	7	NULL	NULL	0	NULL	fibronectin ( alpha 3 beta 1 ) receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These include the well-characterized fibronectin ( alpha 5 beta 1 ) and the multi-specific laminin , collagen and fibronectin ( alpha 3 beta 1 ) receptors .
	manualset3
176260	1	413688	7	NULL	NULL	0	NULL	Addition 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of hydrogen peroxide , diamide , and the superoxide generating agent paraquat to exponentially growing cells revealed complex changes in the protein expression pattern .
	manualset3
176261	2	413688	7	NULL	NULL	0	NULL	hydrogen peroxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of hydrogen peroxide , diamide , and the superoxide generating agent paraquat to exponentially growing cells revealed complex changes in the protein expression pattern .
	manualset3
176262	3	413688	7	NULL	NULL	0	NULL	diamide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of hydrogen peroxide , diamide , and the superoxide generating agent paraquat to exponentially growing cells revealed complex changes in the protein expression pattern .
	manualset3
176263	4	413688	7	NULL	NULL	0	NULL	superoxide generating agent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of hydrogen peroxide , diamide , and the superoxide generating agent paraquat to exponentially growing cells revealed complex changes in the protein expression pattern .
	manualset3
176264	5	413688	7	NULL	NULL	0	NULL	growing cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of hydrogen peroxide , diamide , and the superoxide generating agent paraquat to exponentially growing cells revealed complex changes in the protein expression pattern .
	manualset3
176265	6	413688	7	NULL	NULL	0	NULL	complex changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of hydrogen peroxide , diamide , and the superoxide generating agent paraquat to exponentially growing cells revealed complex changes in the protein expression pattern .
	manualset3
176266	7	413688	7	NULL	NULL	0	NULL	protein expression pattern	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of hydrogen peroxide , diamide , and the superoxide generating agent paraquat to exponentially growing cells revealed complex changes in the protein expression pattern .
	manualset3
176267	1	413689	7	NULL	NULL	0	NULL	impulse-supporting portion	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These included eliminating the impulse-supporting portion of the motor neuron by pinching off its axon , abolishing impulses by replacing Na + with Tris in the medium bathing the nerve cord , and increasing the threshold for impulse production by raising the Mg2 + and Ca2 + concentrations in the medium bathing the nerve cord .
	manualset3
176268	2	413689	7	NULL	NULL	0	NULL	motor neuron	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These included eliminating the impulse-supporting portion of the motor neuron by pinching off its axon , abolishing impulses by replacing Na + with Tris in the medium bathing the nerve cord , and increasing the threshold for impulse production by raising the Mg2 + and Ca2 + concentrations in the medium bathing the nerve cord .
	manualset3
176269	3	413689	7	NULL	NULL	0	NULL	axon	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These included eliminating the impulse-supporting portion of the motor neuron by pinching off its axon , abolishing impulses by replacing Na + with Tris in the medium bathing the nerve cord , and increasing the threshold for impulse production by raising the Mg2 + and Ca2 + concentrations in the medium bathing the nerve cord .
	manualset3
176270	4	413689	7	NULL	NULL	NULL	NULL	Na + 	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These included eliminating the impulse-supporting portion of the motor neuron by pinching off its axon , abolishing impulses by replacing Na + with Tris in the medium bathing the nerve cord , and increasing the threshold for impulse production by raising the Mg2 + and Ca2 + concentrations in the medium bathing the nerve cord .
	manualset3
176271	5	413689	7	NULL	NULL	0	NULL	medium	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These included eliminating the impulse-supporting portion of the motor neuron by pinching off its axon , abolishing impulses by replacing Na + with Tris in the medium bathing the nerve cord , and increasing the threshold for impulse production by raising the Mg2 + and Ca2 + concentrations in the medium bathing the nerve cord .
	manualset3
176272	6	413689	7	NULL	NULL	0	NULL	 nerve cord	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These included eliminating the impulse-supporting portion of the motor neuron by pinching off its axon , abolishing impulses by replacing Na + with Tris in the medium bathing the nerve cord , and increasing the threshold for impulse production by raising the Mg2 + and Ca2 + concentrations in the medium bathing the nerve cord .
	manualset3
176273	7	413689	7	NULL	NULL	0	NULL	threshold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These included eliminating the impulse-supporting portion of the motor neuron by pinching off its axon , abolishing impulses by replacing Na + with Tris in the medium bathing the nerve cord , and increasing the threshold for impulse production by raising the Mg2 + and Ca2 + concentrations in the medium bathing the nerve cord .
	manualset3
176274	8	413689	7	NULL	NULL	0	NULL	impulse production 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These included eliminating the impulse-supporting portion of the motor neuron by pinching off its axon , abolishing impulses by replacing Na + with Tris in the medium bathing the nerve cord , and increasing the threshold for impulse production by raising the Mg2 + and Ca2 + concentrations in the medium bathing the nerve cord .
	manualset3
176275	9	413689	7	NULL	NULL	0	NULL	Mg2 + concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These included eliminating the impulse-supporting portion of the motor neuron by pinching off its axon , abolishing impulses by replacing Na + with Tris in the medium bathing the nerve cord , and increasing the threshold for impulse production by raising the Mg2 + and Ca2 + concentrations in the medium bathing the nerve cord .
	manualset3
176276	10	413689	7	NULL	NULL	0	NULL	 Ca2 + concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These included eliminating the impulse-supporting portion of the motor neuron by pinching off its axon , abolishing impulses by replacing Na + with Tris in the medium bathing the nerve cord , and increasing the threshold for impulse production by raising the Mg2 + and Ca2 + concentrations in the medium bathing the nerve cord .
	manualset3
176277	11	413689	7	NULL	NULL	0	NULL	medium	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These included eliminating the impulse-supporting portion of the motor neuron by pinching off its axon , abolishing impulses by replacing Na + with Tris in the medium bathing the nerve cord , and increasing the threshold for impulse production by raising the Mg2 + and Ca2 + concentrations in the medium bathing the nerve cord .
	manualset3
176278	12	413689	7	NULL	NULL	0	NULL	nerve cord	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These included eliminating the impulse-supporting portion of the motor neuron by pinching off its axon , abolishing impulses by replacing Na + with Tris in the medium bathing the nerve cord , and increasing the threshold for impulse production by raising the Mg2 + and Ca2 + concentrations in the medium bathing the nerve cord .
	manualset3
178200	13	413689	7	NULL	NULL	0	NULL	 impulses 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These included eliminating the impulse-supporting portion of the motor neuron by pinching off its axon , abolishing impulses by replacing Na + with Tris in the medium bathing the nerve cord , and increasing the threshold for impulse production by raising the Mg2 + and Ca2 + concentrations in the medium bathing the nerve cord .
	manualset3
178886	14	413689	7	NULL	NULL	0	NULL	Tris	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These included eliminating the impulse-supporting portion of the motor neuron by pinching off its axon , abolishing impulses by replacing Na + with Tris in the medium bathing the nerve cord , and increasing the threshold for impulse production by raising the Mg2 + and Ca2 + concentrations in the medium bathing the nerve cord .
	manualset3
178888	15	413689	7	NULL	NULL	0	NULL	 eliminating	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These included eliminating the impulse-supporting portion of the motor neuron by pinching off its axon , abolishing impulses by replacing Na + with Tris in the medium bathing the nerve cord , and increasing the threshold for impulse production by raising the Mg2 + and Ca2 + concentrations in the medium bathing the nerve cord .
	manualset3
178889	16	413689	7	NULL	NULL	0	NULL	pinching off	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These included eliminating the impulse-supporting portion of the motor neuron by pinching off its axon , abolishing impulses by replacing Na + with Tris in the medium bathing the nerve cord , and increasing the threshold for impulse production by raising the Mg2 + and Ca2 + concentrations in the medium bathing the nerve cord .
	manualset3
178890	17	413689	7	NULL	NULL	0	NULL	abolishing impulses	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These included eliminating the impulse-supporting portion of the motor neuron by pinching off its axon , abolishing impulses by replacing Na + with Tris in the medium bathing the nerve cord , and increasing the threshold for impulse production by raising the Mg2 + and Ca2 + concentrations in the medium bathing the nerve cord .
	manualset3
178891	18	413689	7	NULL	NULL	0	NULL	 increasing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These included eliminating the impulse-supporting portion of the motor neuron by pinching off its axon , abolishing impulses by replacing Na + with Tris in the medium bathing the nerve cord , and increasing the threshold for impulse production by raising the Mg2 + and Ca2 + concentrations in the medium bathing the nerve cord .
	manualset3
178892	19	413689	7	NULL	NULL	0	NULL	 raising 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These included eliminating the impulse-supporting portion of the motor neuron by pinching off its axon , abolishing impulses by replacing Na + with Tris in the medium bathing the nerve cord , and increasing the threshold for impulse production by raising the Mg2 + and Ca2 + concentrations in the medium bathing the nerve cord .
	manualset3
178893	20	413689	7	NULL	NULL	NULL	NULL	replacing	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These included eliminating the impulse-supporting portion of the motor neuron by pinching off its axon , abolishing impulses by replacing Na + with Tris in the medium bathing the nerve cord , and increasing the threshold for impulse production by raising the Mg2 + and Ca2 + concentrations in the medium bathing the nerve cord .
	manualset3
176279	1	413690	7	NULL	NULL	0	NULL	older age	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	These included older age ( 55.2 % ) 60 years , 20.6 % ) 70 years ) , immigration to Israel during the preceding 5 years ( 34.7 % ) , concomitant physical illness ( 60 % ) which was associated with moderate to severe disability in 41 % and poor quality of antidepressant pharmacotherapy prior to hospitalisation ( only 24.3 % received an adequate trial of antidepressant medication ) .
	manualset3
176280	2	413690	7	NULL	NULL	0	NULL	55.2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These included older age ( 55.2 % ) 60 years , 20.6 % ) 70 years ) , immigration to Israel during the preceding 5 years ( 34.7 % ) , concomitant physical illness ( 60 % ) which was associated with moderate to severe disability in 41 % and poor quality of antidepressant pharmacotherapy prior to hospitalisation ( only 24.3 % received an adequate trial of antidepressant medication ) .
	manualset3
176281	3	413690	7	NULL	NULL	0	NULL	60 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	These included older age ( 55.2 % ) 60 years , 20.6 % ) 70 years ) , immigration to Israel during the preceding 5 years ( 34.7 % ) , concomitant physical illness ( 60 % ) which was associated with moderate to severe disability in 41 % and poor quality of antidepressant pharmacotherapy prior to hospitalisation ( only 24.3 % received an adequate trial of antidepressant medication ) .
	manualset3
176282	4	413690	7	NULL	NULL	0	NULL	20.6 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These included older age ( 55.2 % ) 60 years , 20.6 % ) 70 years ) , immigration to Israel during the preceding 5 years ( 34.7 % ) , concomitant physical illness ( 60 % ) which was associated with moderate to severe disability in 41 % and poor quality of antidepressant pharmacotherapy prior to hospitalisation ( only 24.3 % received an adequate trial of antidepressant medication ) .
	manualset3
176283	5	413690	7	NULL	NULL	0	NULL	70 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	These included older age ( 55.2 % ) 60 years , 20.6 % ) 70 years ) , immigration to Israel during the preceding 5 years ( 34.7 % ) , concomitant physical illness ( 60 % ) which was associated with moderate to severe disability in 41 % and poor quality of antidepressant pharmacotherapy prior to hospitalisation ( only 24.3 % received an adequate trial of antidepressant medication ) .
	manualset3
176284	6	413690	7	NULL	NULL	0	NULL	 immigration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These included older age ( 55.2 % ) 60 years , 20.6 % ) 70 years ) , immigration to Israel during the preceding 5 years ( 34.7 % ) , concomitant physical illness ( 60 % ) which was associated with moderate to severe disability in 41 % and poor quality of antidepressant pharmacotherapy prior to hospitalisation ( only 24.3 % received an adequate trial of antidepressant medication ) .
	manualset3
176285	7	413690	7	NULL	NULL	0	NULL	Israel 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	These included older age ( 55.2 % ) 60 years , 20.6 % ) 70 years ) , immigration to Israel during the preceding 5 years ( 34.7 % ) , concomitant physical illness ( 60 % ) which was associated with moderate to severe disability in 41 % and poor quality of antidepressant pharmacotherapy prior to hospitalisation ( only 24.3 % received an adequate trial of antidepressant medication ) .
	manualset3
176286	8	413690	7	NULL	NULL	0	NULL	5 years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	These included older age ( 55.2 % ) 60 years , 20.6 % ) 70 years ) , immigration to Israel during the preceding 5 years ( 34.7 % ) , concomitant physical illness ( 60 % ) which was associated with moderate to severe disability in 41 % and poor quality of antidepressant pharmacotherapy prior to hospitalisation ( only 24.3 % received an adequate trial of antidepressant medication ) .
	manualset3
176287	9	413690	7	NULL	NULL	0	NULL	34.7 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These included older age ( 55.2 % ) 60 years , 20.6 % ) 70 years ) , immigration to Israel during the preceding 5 years ( 34.7 % ) , concomitant physical illness ( 60 % ) which was associated with moderate to severe disability in 41 % and poor quality of antidepressant pharmacotherapy prior to hospitalisation ( only 24.3 % received an adequate trial of antidepressant medication ) .
	manualset3
176288	10	413690	7	NULL	NULL	0	NULL	 concomitant physical illness 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These included older age ( 55.2 % ) 60 years , 20.6 % ) 70 years ) , immigration to Israel during the preceding 5 years ( 34.7 % ) , concomitant physical illness ( 60 % ) which was associated with moderate to severe disability in 41 % and poor quality of antidepressant pharmacotherapy prior to hospitalisation ( only 24.3 % received an adequate trial of antidepressant medication ) .
	manualset3
176289	11	413690	7	NULL	NULL	0	NULL	60 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These included older age ( 55.2 % ) 60 years , 20.6 % ) 70 years ) , immigration to Israel during the preceding 5 years ( 34.7 % ) , concomitant physical illness ( 60 % ) which was associated with moderate to severe disability in 41 % and poor quality of antidepressant pharmacotherapy prior to hospitalisation ( only 24.3 % received an adequate trial of antidepressant medication ) .
	manualset3
176290	12	413690	7	NULL	NULL	0	NULL	moderate disability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These included older age ( 55.2 % ) 60 years , 20.6 % ) 70 years ) , immigration to Israel during the preceding 5 years ( 34.7 % ) , concomitant physical illness ( 60 % ) which was associated with moderate to severe disability in 41 % and poor quality of antidepressant pharmacotherapy prior to hospitalisation ( only 24.3 % received an adequate trial of antidepressant medication ) .
	manualset3
176291	13	413690	7	NULL	NULL	0	NULL	severe disability 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These included older age ( 55.2 % ) 60 years , 20.6 % ) 70 years ) , immigration to Israel during the preceding 5 years ( 34.7 % ) , concomitant physical illness ( 60 % ) which was associated with moderate to severe disability in 41 % and poor quality of antidepressant pharmacotherapy prior to hospitalisation ( only 24.3 % received an adequate trial of antidepressant medication ) .
	manualset3
176292	14	413690	7	NULL	NULL	0	NULL	41 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These included older age ( 55.2 % ) 60 years , 20.6 % ) 70 years ) , immigration to Israel during the preceding 5 years ( 34.7 % ) , concomitant physical illness ( 60 % ) which was associated with moderate to severe disability in 41 % and poor quality of antidepressant pharmacotherapy prior to hospitalisation ( only 24.3 % received an adequate trial of antidepressant medication ) .
	manualset3
176293	15	413690	7	NULL	NULL	0	NULL	poor quality 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These included older age ( 55.2 % ) 60 years , 20.6 % ) 70 years ) , immigration to Israel during the preceding 5 years ( 34.7 % ) , concomitant physical illness ( 60 % ) which was associated with moderate to severe disability in 41 % and poor quality of antidepressant pharmacotherapy prior to hospitalisation ( only 24.3 % received an adequate trial of antidepressant medication ) .
	manualset3
176294	16	413690	7	NULL	NULL	0	NULL	antidepressant pharmacotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These included older age ( 55.2 % ) 60 years , 20.6 % ) 70 years ) , immigration to Israel during the preceding 5 years ( 34.7 % ) , concomitant physical illness ( 60 % ) which was associated with moderate to severe disability in 41 % and poor quality of antidepressant pharmacotherapy prior to hospitalisation ( only 24.3 % received an adequate trial of antidepressant medication ) .
	manualset3
176295	17	413690	7	NULL	NULL	NULL	NULL	 hospitalisation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These included older age ( 55.2 % ) 60 years , 20.6 % ) 70 years ) , immigration to Israel during the preceding 5 years ( 34.7 % ) , concomitant physical illness ( 60 % ) which was associated with moderate to severe disability in 41 % and poor quality of antidepressant pharmacotherapy prior to hospitalisation ( only 24.3 % received an adequate trial of antidepressant medication ) .
	manualset3
176296	18	413690	7	NULL	NULL	0	NULL	24.3 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These included older age ( 55.2 % ) 60 years , 20.6 % ) 70 years ) , immigration to Israel during the preceding 5 years ( 34.7 % ) , concomitant physical illness ( 60 % ) which was associated with moderate to severe disability in 41 % and poor quality of antidepressant pharmacotherapy prior to hospitalisation ( only 24.3 % received an adequate trial of antidepressant medication ) .
	manualset3
176297	19	413690	7	NULL	NULL	0	NULL	trial	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These included older age ( 55.2 % ) 60 years , 20.6 % ) 70 years ) , immigration to Israel during the preceding 5 years ( 34.7 % ) , concomitant physical illness ( 60 % ) which was associated with moderate to severe disability in 41 % and poor quality of antidepressant pharmacotherapy prior to hospitalisation ( only 24.3 % received an adequate trial of antidepressant medication ) .
	manualset3
176298	20	413690	7	NULL	NULL	0	NULL	 antidepressant medication 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These included older age ( 55.2 % ) 60 years , 20.6 % ) 70 years ) , immigration to Israel during the preceding 5 years ( 34.7 % ) , concomitant physical illness ( 60 % ) which was associated with moderate to severe disability in 41 % and poor quality of antidepressant pharmacotherapy prior to hospitalisation ( only 24.3 % received an adequate trial of antidepressant medication ) .
	manualset3
178201	1	413691	7	NULL	NULL	0	NULL	over-expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These included over-expression of antisense mu-calpain ( mu-AS ) , dominant negative mu-calpain ( mu-DN ) and the antisense 30-kDa calpain subunit ( 30-AS ) .
	manualset3
178202	2	413691	7	NULL	NULL	NULL	NULL	antisense mu-calpain ( mu-AS )	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These included over-expression of antisense mu-calpain ( mu-AS ) , dominant negative mu-calpain ( mu-DN ) and the antisense 30-kDa calpain subunit ( 30-AS ) .
	manualset3
178203	3	413691	7	NULL	NULL	0	NULL	dominant negative mu-calpain ( mu-DN )	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These included over-expression of antisense mu-calpain ( mu-AS ) , dominant negative mu-calpain ( mu-DN ) and the antisense 30-kDa calpain subunit ( 30-AS ) .
	manualset3
178204	4	413691	7	NULL	NULL	0	NULL	antisense 30-kDa calpain subunit ( 30-AS )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These included over-expression of antisense mu-calpain ( mu-AS ) , dominant negative mu-calpain ( mu-DN ) and the antisense 30-kDa calpain subunit ( 30-AS ) .
	manualset3
178205	1	413692	7	NULL	NULL	0	NULL	chewing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These increases demonstrate that chewing activates widespread regions of the brain .
	manualset3
178206	2	413692	7	NULL	NULL	0	NULL	widespread regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These increases demonstrate that chewing activates widespread regions of the brain .
	manualset3
178207	3	413692	7	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These increases demonstrate that chewing activates widespread regions of the brain .
	manualset3
178208	1	413693	7	NULL	NULL	0	NULL	individuals 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These individuals initially found the procedure difficult to comprehend because they could not easily visualize past anger-producing situations , but mastery was achieved when we incorporated recreating-the-scene as a prompt and added a discriminative stimulus on the soles of the participants ' feet .
	manualset3
178209	2	413693	7	NULL	NULL	0	NULL	procedure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These individuals initially found the procedure difficult to comprehend because they could not easily visualize past anger-producing situations , but mastery was achieved when we incorporated recreating-the-scene as a prompt and added a discriminative stimulus on the soles of the participants ' feet .
	manualset3
178210	3	413693	7	NULL	NULL	0	NULL	past anger-producing situations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These individuals initially found the procedure difficult to comprehend because they could not easily visualize past anger-producing situations , but mastery was achieved when we incorporated recreating-the-scene as a prompt and added a discriminative stimulus on the soles of the participants ' feet .
	manualset3
178211	4	413693	7	NULL	NULL	0	NULL	mastery	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These individuals initially found the procedure difficult to comprehend because they could not easily visualize past anger-producing situations , but mastery was achieved when we incorporated recreating-the-scene as a prompt and added a discriminative stimulus on the soles of the participants ' feet .
	manualset3
178212	5	413693	7	NULL	NULL	0	NULL	recreating-the-scene	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These individuals initially found the procedure difficult to comprehend because they could not easily visualize past anger-producing situations , but mastery was achieved when we incorporated recreating-the-scene as a prompt and added a discriminative stimulus on the soles of the participants ' feet .
	manualset3
178213	6	413693	7	NULL	NULL	0	NULL	stimulus	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These individuals initially found the procedure difficult to comprehend because they could not easily visualize past anger-producing situations , but mastery was achieved when we incorporated recreating-the-scene as a prompt and added a discriminative stimulus on the soles of the participants ' feet .
	manualset3
178214	7	413693	7	NULL	NULL	0	NULL	soles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These individuals initially found the procedure difficult to comprehend because they could not easily visualize past anger-producing situations , but mastery was achieved when we incorporated recreating-the-scene as a prompt and added a discriminative stimulus on the soles of the participants ' feet .
	manualset3
178215	8	413693	7	NULL	NULL	0	NULL	participants ' feet	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These individuals initially found the procedure difficult to comprehend because they could not easily visualize past anger-producing situations , but mastery was achieved when we incorporated recreating-the-scene as a prompt and added a discriminative stimulus on the soles of the participants ' feet .
	manualset3
178216	1	413694	7	NULL	NULL	NULL	NULL	inhibitors	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These inhibitors also enhanced the sucrose starvation-induced accumulation of alphaAmy3 mRNA but not that of alphaAmy7 or alphaAmy8 mRNAs .
	manualset3
178217	2	413694	7	NULL	NULL	0	NULL	sucrose starvation-induced accumulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These inhibitors also enhanced the sucrose starvation-induced accumulation of alphaAmy3 mRNA but not that of alphaAmy7 or alphaAmy8 mRNAs .
	manualset3
178218	3	413694	7	NULL	NULL	0	NULL	alphaAmy3 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These inhibitors also enhanced the sucrose starvation-induced accumulation of alphaAmy3 mRNA but not that of alphaAmy7 or alphaAmy8 mRNAs .
	manualset3
178219	4	413694	7	NULL	NULL	0	NULL	alphaAmy7 mRNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These inhibitors also enhanced the sucrose starvation-induced accumulation of alphaAmy3 mRNA but not that of alphaAmy7 or alphaAmy8 mRNAs .
	manualset3
178220	5	413694	7	NULL	NULL	0	NULL	alphaAmy8 mRNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These inhibitors also enhanced the sucrose starvation-induced accumulation of alphaAmy3 mRNA but not that of alphaAmy7 or alphaAmy8 mRNAs .
	manualset3
178221	1	413695	7	NULL	NULL	0	NULL	actions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These inhibitory and potentiating actions of 5-hydroxytryptamine were reversed by cyproheptadine and 2-bromolysergic acid diethylamide .
	manualset3
178222	2	413695	7	NULL	NULL	0	NULL	5-hydroxytryptamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These inhibitory and potentiating actions of 5-hydroxytryptamine were reversed by cyproheptadine and 2-bromolysergic acid diethylamide .
	manualset3
178223	3	413695	7	NULL	NULL	0	NULL	cyproheptadine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These inhibitory and potentiating actions of 5-hydroxytryptamine were reversed by cyproheptadine and 2-bromolysergic acid diethylamide .
	manualset3
178224	4	413695	7	NULL	NULL	0	NULL	2-bromolysergic acid diethylamide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These inhibitory and potentiating actions of 5-hydroxytryptamine were reversed by cyproheptadine and 2-bromolysergic acid diethylamide .
	manualset3
178225	1	413696	7	NULL	NULL	0	NULL	 interactions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These interactions activate many intracellular signaling pathways that regulate processes such as cell adhesion , migration , and survival .
	manualset3
178226	2	413696	7	NULL	NULL	0	NULL	intracellular signaling pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These interactions activate many intracellular signaling pathways that regulate processes such as cell adhesion , migration , and survival .
	manualset3
178227	3	413696	7	NULL	NULL	0	NULL	cell adhesion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These interactions activate many intracellular signaling pathways that regulate processes such as cell adhesion , migration , and survival .
	manualset3
178228	4	413696	7	NULL	NULL	0	NULL	cell migration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These interactions activate many intracellular signaling pathways that regulate processes such as cell adhesion , migration , and survival .
	manualset3
178229	5	413696	7	NULL	NULL	0	NULL	cell survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These interactions activate many intracellular signaling pathways that regulate processes such as cell adhesion , migration , and survival .
	manualset3
190513	6	413696	7	NULL	NULL	0	NULL	processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These interactions activate many intracellular signaling pathways that regulate processes such as cell adhesion , migration , and survival .
	manualset3
178230	1	413697	7	NULL	NULL	0	NULL	 interdomain contacts	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These interdomain contacts provide a functional explanation for how PIP ( 2 ) binding and tyrosine phosphorylation of ezrin lead to activation , and provide an understanding of previously enigmatic loss-of-function missense mutations in the tumor suppressor merlin .
	manualset3
178231	2	413697	7	NULL	NULL	0	NULL	functional explanation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These interdomain contacts provide a functional explanation for how PIP ( 2 ) binding and tyrosine phosphorylation of ezrin lead to activation , and provide an understanding of previously enigmatic loss-of-function missense mutations in the tumor suppressor merlin .
	manualset3
178232	3	413697	7	NULL	NULL	0	NULL	PIP ( 2 ) binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These interdomain contacts provide a functional explanation for how PIP ( 2 ) binding and tyrosine phosphorylation of ezrin lead to activation , and provide an understanding of previously enigmatic loss-of-function missense mutations in the tumor suppressor merlin .
	manualset3
178233	4	413697	7	NULL	NULL	0	NULL	tyrosine phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These interdomain contacts provide a functional explanation for how PIP ( 2 ) binding and tyrosine phosphorylation of ezrin lead to activation , and provide an understanding of previously enigmatic loss-of-function missense mutations in the tumor suppressor merlin .
	manualset3
178234	5	413697	7	NULL	NULL	0	NULL	ezrin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These interdomain contacts provide a functional explanation for how PIP ( 2 ) binding and tyrosine phosphorylation of ezrin lead to activation , and provide an understanding of previously enigmatic loss-of-function missense mutations in the tumor suppressor merlin .
	manualset3
178235	6	413697	7	NULL	NULL	NULL	NULL	activation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These interdomain contacts provide a functional explanation for how PIP ( 2 ) binding and tyrosine phosphorylation of ezrin lead to activation , and provide an understanding of previously enigmatic loss-of-function missense mutations in the tumor suppressor merlin .
	manualset3
178236	7	413697	7	NULL	NULL	NULL	NULL	 loss-of-function	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These interdomain contacts provide a functional explanation for how PIP ( 2 ) binding and tyrosine phosphorylation of ezrin lead to activation , and provide an understanding of previously enigmatic loss-of-function missense mutations in the tumor suppressor merlin .
	manualset3
178237	8	413697	7	NULL	NULL	0	NULL	missense mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These interdomain contacts provide a functional explanation for how PIP ( 2 ) binding and tyrosine phosphorylation of ezrin lead to activation , and provide an understanding of previously enigmatic loss-of-function missense mutations in the tumor suppressor merlin .
	manualset3
178238	9	413697	7	NULL	NULL	0	NULL	tumor suppressor merlin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These interdomain contacts provide a functional explanation for how PIP ( 2 ) binding and tyrosine phosphorylation of ezrin lead to activation , and provide an understanding of previously enigmatic loss-of-function missense mutations in the tumor suppressor merlin .
	manualset3
190514	10	413697	7	NULL	NULL	0	NULL	understanding 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These interdomain contacts provide a functional explanation for how PIP ( 2 ) binding and tyrosine phosphorylation of ezrin lead to activation , and provide an understanding of previously enigmatic loss-of-function missense mutations in the tumor suppressor merlin .
	manualset3
178239	1	413698	7	NULL	NULL	0	NULL	Addition 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of polyamines or basic amino acids which are known to be sequestered in vacuoles did not effect polyphosphate metabolism .
	manualset3
178240	2	413698	7	NULL	NULL	NULL	NULL	polyamines	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Addition of polyamines or basic amino acids which are known to be sequestered in vacuoles did not effect polyphosphate metabolism .
	manualset3
178241	3	413698	7	NULL	NULL	0	NULL	basic amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of polyamines or basic amino acids which are known to be sequestered in vacuoles did not effect polyphosphate metabolism .
	manualset3
178242	4	413698	7	NULL	NULL	0	NULL	vacuoles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of polyamines or basic amino acids which are known to be sequestered in vacuoles did not effect polyphosphate metabolism .
	manualset3
178243	5	413698	7	NULL	NULL	0	NULL	polyphosphate metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of polyamines or basic amino acids which are known to be sequestered in vacuoles did not effect polyphosphate metabolism .
	manualset3
178244	1	413699	7	NULL	NULL	0	NULL	internalized vesicles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These internalized vesicles may shuttle back to the plasma membrane to recycle the membrane components or they may be targeted for degradation .
	manualset3
178245	2	413699	7	NULL	NULL	0	NULL	plasma membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These internalized vesicles may shuttle back to the plasma membrane to recycle the membrane components or they may be targeted for degradation .
	manualset3
178246	3	413699	7	NULL	NULL	0	NULL	membrane components	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These internalized vesicles may shuttle back to the plasma membrane to recycle the membrane components or they may be targeted for degradation .
	manualset3
178247	4	413699	7	NULL	NULL	0	NULL	degradation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These internalized vesicles may shuttle back to the plasma membrane to recycle the membrane components or they may be targeted for degradation .
	manualset3
176359	1	413700	7	NULL	NULL	0	NULL	interventions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These interventions include reperfusion , a variety of pharmacological agents , and physical and hemodynamic interventions .
	manualset3
176360	2	413700	7	NULL	NULL	0	NULL	reperfusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These interventions include reperfusion , a variety of pharmacological agents , and physical and hemodynamic interventions .
	manualset3
176361	3	413700	7	NULL	NULL	0	NULL	pharmacological agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These interventions include reperfusion , a variety of pharmacological agents , and physical and hemodynamic interventions .
	manualset3
176362	4	413700	7	NULL	NULL	0	NULL	physical interventions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These interventions include reperfusion , a variety of pharmacological agents , and physical and hemodynamic interventions .
	manualset3
176363	5	413700	7	NULL	NULL	0	NULL	hemodynamic interventions 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These interventions include reperfusion , a variety of pharmacological agents , and physical and hemodynamic interventions .
	manualset3
176364	1	413701	7	NULL	NULL	0	NULL	large microspheres 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These large microspheres ( ) 100 microm ) can be employed in the mesofluidic systems for automated heterogeneous assays .
	manualset3
176365	2	413701	7	NULL	NULL	0	NULL	100 microm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These large microspheres ( ) 100 microm ) can be employed in the mesofluidic systems for automated heterogeneous assays .
	manualset3
176366	3	413701	7	NULL	NULL	0	NULL	mesofluidic systems	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These large microspheres ( ) 100 microm ) can be employed in the mesofluidic systems for automated heterogeneous assays .
	manualset3
176367	4	413701	7	NULL	NULL	0	NULL	 automated heterogeneous assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These large microspheres ( ) 100 microm ) can be employed in the mesofluidic systems for automated heterogeneous assays .
	manualset3
176368	1	413702	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These later data may be of value for a more rational therapeutic approach of the paroxysmal arrhythmias in the WPW syndrome .
	manualset3
176369	2	413702	7	NULL	NULL	0	NULL	value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These later data may be of value for a more rational therapeutic approach of the paroxysmal arrhythmias in the WPW syndrome .
	manualset3
176370	3	413702	7	NULL	NULL	0	NULL	rational therapeutic approach 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These later data may be of value for a more rational therapeutic approach of the paroxysmal arrhythmias in the WPW syndrome .
	manualset3
176371	4	413702	7	NULL	NULL	0	NULL	paroxysmal arrhythmias	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These later data may be of value for a more rational therapeutic approach of the paroxysmal arrhythmias in the WPW syndrome .
	manualset3
176372	5	413702	7	NULL	NULL	0	NULL	WPW syndrome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These later data may be of value for a more rational therapeutic approach of the paroxysmal arrhythmias in the WPW syndrome .
	manualset3
176373	1	413703	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These latter results show that the respiratory and behavioral effects of beta-CCE in rhesus monkeys are at least in part due to effects at BZRs .
	manualset3
176374	2	413703	7	NULL	NULL	0	NULL	respiratory effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These latter results show that the respiratory and behavioral effects of beta-CCE in rhesus monkeys are at least in part due to effects at BZRs .
	manualset3
176375	3	413703	7	NULL	NULL	0	NULL	behavioral effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These latter results show that the respiratory and behavioral effects of beta-CCE in rhesus monkeys are at least in part due to effects at BZRs .
	manualset3
176376	4	413703	7	NULL	NULL	0	NULL	beta-CCE	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These latter results show that the respiratory and behavioral effects of beta-CCE in rhesus monkeys are at least in part due to effects at BZRs .
	manualset3
176377	5	413703	7	NULL	NULL	0	NULL	rhesus monkeys	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These latter results show that the respiratory and behavioral effects of beta-CCE in rhesus monkeys are at least in part due to effects at BZRs .
	manualset3
176378	6	413703	7	NULL	NULL	0	NULL	BZRs 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These latter results show that the respiratory and behavioral effects of beta-CCE in rhesus monkeys are at least in part due to effects at BZRs .
	manualset3
176379	7	413703	7	NULL	NULL	0	NULL	effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These latter results show that the respiratory and behavioral effects of beta-CCE in rhesus monkeys are at least in part due to effects at BZRs .
	manualset3
176380	1	413704	7	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These lead to significant differences in rise time and activation times between the optically acquired calcium signal and the epicardial intracellular calcium concentration .
	manualset3
176381	2	413704	7	NULL	NULL	0	NULL	rise time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	These lead to significant differences in rise time and activation times between the optically acquired calcium signal and the epicardial intracellular calcium concentration .
	manualset3
176382	3	413704	7	NULL	NULL	0	NULL	activation times	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	These lead to significant differences in rise time and activation times between the optically acquired calcium signal and the epicardial intracellular calcium concentration .
	manualset3
176383	4	413704	7	NULL	NULL	0	NULL	optically acquired calcium signal	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These lead to significant differences in rise time and activation times between the optically acquired calcium signal and the epicardial intracellular calcium concentration .
	manualset3
176384	5	413704	7	NULL	NULL	0	NULL	epicardial intracellular calcium concentration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These lead to significant differences in rise time and activation times between the optically acquired calcium signal and the epicardial intracellular calcium concentration .
	manualset3
176385	1	413705	7	NULL	NULL	0	NULL	 leukemias	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These leukemias are characterized by the presence of blasts , which express CD56 , in the peripheral blood , bone marrow , lymph nodes , and/or extranodal tissues .
	manualset3
176386	2	413705	7	NULL	NULL	0	NULL	presence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These leukemias are characterized by the presence of blasts , which express CD56 , in the peripheral blood , bone marrow , lymph nodes , and/or extranodal tissues .
	manualset3
176387	3	413705	7	NULL	NULL	0	NULL	blasts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These leukemias are characterized by the presence of blasts , which express CD56 , in the peripheral blood , bone marrow , lymph nodes , and/or extranodal tissues .
	manualset3
176388	4	413705	7	NULL	NULL	0	NULL	CD56	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These leukemias are characterized by the presence of blasts , which express CD56 , in the peripheral blood , bone marrow , lymph nodes , and/or extranodal tissues .
	manualset3
176389	5	413705	7	NULL	NULL	0	NULL	peripheral blood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These leukemias are characterized by the presence of blasts , which express CD56 , in the peripheral blood , bone marrow , lymph nodes , and/or extranodal tissues .
	manualset3
176390	6	413705	7	NULL	NULL	0	NULL	bone marrow	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These leukemias are characterized by the presence of blasts , which express CD56 , in the peripheral blood , bone marrow , lymph nodes , and/or extranodal tissues .
	manualset3
176391	7	413705	7	NULL	NULL	0	NULL	lymph nodes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These leukemias are characterized by the presence of blasts , which express CD56 , in the peripheral blood , bone marrow , lymph nodes , and/or extranodal tissues .
	manualset3
176392	8	413705	7	NULL	NULL	0	NULL	extranodal tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	These leukemias are characterized by the presence of blasts , which express CD56 , in the peripheral blood , bone marrow , lymph nodes , and/or extranodal tissues .
	manualset3
176393	1	413706	7	NULL	NULL	0	NULL	Addition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of polyclonal mitogen ( E. coli lipopolysaccharide ) at 10 micrograms/ml markedly increased the production of hybridomas secreting anti-urease , but most were of IgM class .
	manualset3
176394	2	413706	7	NULL	NULL	0	NULL	polyclonal mitogen ( E. coli lipopolysaccharide )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of polyclonal mitogen ( E. coli lipopolysaccharide ) at 10 micrograms/ml markedly increased the production of hybridomas secreting anti-urease , but most were of IgM class .
	manualset3
176395	3	413706	7	NULL	NULL	0	NULL	 10 micrograms/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of polyclonal mitogen ( E. coli lipopolysaccharide ) at 10 micrograms/ml markedly increased the production of hybridomas secreting anti-urease , but most were of IgM class .
	manualset3
176396	4	413706	7	NULL	NULL	0	NULL	production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of polyclonal mitogen ( E. coli lipopolysaccharide ) at 10 micrograms/ml markedly increased the production of hybridomas secreting anti-urease , but most were of IgM class .
	manualset3
176397	5	413706	7	NULL	NULL	NULL	NULL	hybridomas secreting anti-urease	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Addition of polyclonal mitogen ( E. coli lipopolysaccharide ) at 10 micrograms/ml markedly increased the production of hybridomas secreting anti-urease , but most were of IgM class .
	manualset3
176398	6	413706	7	NULL	NULL	0	NULL	IgM class	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of polyclonal mitogen ( E. coli lipopolysaccharide ) at 10 micrograms/ml markedly increased the production of hybridomas secreting anti-urease , but most were of IgM class .
	manualset3
176399	1	413707	7	NULL	NULL	0	NULL	livers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These livers were less efficient in converting AFB1 to a mutagen , when compared to control S20 .
	manualset3
176400	2	413707	7	NULL	NULL	0	NULL	AFB1	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These livers were less efficient in converting AFB1 to a mutagen , when compared to control S20 .
	manualset3
176401	3	413707	7	NULL	NULL	0	NULL	mutagen	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These livers were less efficient in converting AFB1 to a mutagen , when compared to control S20 .
	manualset3
176402	4	413707	7	NULL	NULL	0	NULL	control S20	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These livers were less efficient in converting AFB1 to a mutagen , when compared to control S20 .
	manualset3
176989	1	413708	7	NULL	NULL	0	NULL	macromolecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	These macromolecules probably enter the lysosome-like bodies by a crino-phagic mechanism , i.e. , fusion of these organelles with the apical vesicles and tubules involved in intracellular transport .
	manualset3
176990	2	413708	7	NULL	NULL	0	NULL	lysosome-like bodies	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These macromolecules probably enter the lysosome-like bodies by a crino-phagic mechanism , i.e. , fusion of these organelles with the apical vesicles and tubules involved in intracellular transport .
	manualset3
176991	3	413708	7	NULL	NULL	0	NULL	crino-phagic mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These macromolecules probably enter the lysosome-like bodies by a crino-phagic mechanism , i.e. , fusion of these organelles with the apical vesicles and tubules involved in intracellular transport .
	manualset3
176992	4	413708	7	NULL	NULL	0	NULL	fusion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These macromolecules probably enter the lysosome-like bodies by a crino-phagic mechanism , i.e. , fusion of these organelles with the apical vesicles and tubules involved in intracellular transport .
	manualset3
176993	5	413708	7	NULL	NULL	0	NULL	organelles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These macromolecules probably enter the lysosome-like bodies by a crino-phagic mechanism , i.e. , fusion of these organelles with the apical vesicles and tubules involved in intracellular transport .
	manualset3
176994	6	413708	7	NULL	NULL	0	NULL	apical vesicles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These macromolecules probably enter the lysosome-like bodies by a crino-phagic mechanism , i.e. , fusion of these organelles with the apical vesicles and tubules involved in intracellular transport .
	manualset3
176995	7	413708	7	NULL	NULL	0	NULL	tubules	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These macromolecules probably enter the lysosome-like bodies by a crino-phagic mechanism , i.e. , fusion of these organelles with the apical vesicles and tubules involved in intracellular transport .
	manualset3
176996	8	413708	7	NULL	NULL	NULL	NULL	intracellular transport 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These macromolecules probably enter the lysosome-like bodies by a crino-phagic mechanism , i.e. , fusion of these organelles with the apical vesicles and tubules involved in intracellular transport .
	manualset3
176997	1	413709	7	NULL	NULL	0	NULL	markers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These markers and TEM data differentiate TCs from both satellite cells ( e.g. TCs are Pax7 negative ) and fibroblasts ( which are c-kit negative ) .
	manualset3
176998	2	413709	7	NULL	NULL	0	NULL	TEM data	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These markers and TEM data differentiate TCs from both satellite cells ( e.g. TCs are Pax7 negative ) and fibroblasts ( which are c-kit negative ) .
	manualset3
176999	3	413709	7	NULL	NULL	0	NULL	TCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These markers and TEM data differentiate TCs from both satellite cells ( e.g. TCs are Pax7 negative ) and fibroblasts ( which are c-kit negative ) .
	manualset3
177000	4	413709	7	NULL	NULL	0	NULL	satellite cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These markers and TEM data differentiate TCs from both satellite cells ( e.g. TCs are Pax7 negative ) and fibroblasts ( which are c-kit negative ) .
	manualset3
177001	5	413709	7	NULL	NULL	0	NULL	TCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These markers and TEM data differentiate TCs from both satellite cells ( e.g. TCs are Pax7 negative ) and fibroblasts ( which are c-kit negative ) .
	manualset3
177002	6	413709	7	NULL	NULL	0	NULL	Pax7 negative	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These markers and TEM data differentiate TCs from both satellite cells ( e.g. TCs are Pax7 negative ) and fibroblasts ( which are c-kit negative ) .
	manualset3
177003	7	413709	7	NULL	NULL	0	NULL	fibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These markers and TEM data differentiate TCs from both satellite cells ( e.g. TCs are Pax7 negative ) and fibroblasts ( which are c-kit negative ) .
	manualset3
177004	8	413709	7	NULL	NULL	0	NULL	c-kit negative	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These markers and TEM data differentiate TCs from both satellite cells ( e.g. TCs are Pax7 negative ) and fibroblasts ( which are c-kit negative ) .
	manualset3
177005	1	413710	7	NULL	NULL	NULL	NULL	 measurements	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These measurements of radical density and spatial extent provide the first direct experimental determination of track characteristics in irradiated DNA .
	manualset3
177006	2	413710	7	NULL	NULL	0	NULL	radical density	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These measurements of radical density and spatial extent provide the first direct experimental determination of track characteristics in irradiated DNA .
	manualset3
177007	3	413710	7	NULL	NULL	0	NULL	spatial extent	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These measurements of radical density and spatial extent provide the first direct experimental determination of track characteristics in irradiated DNA .
	manualset3
177008	4	413710	7	NULL	NULL	0	NULL	first direct experimental determination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These measurements of radical density and spatial extent provide the first direct experimental determination of track characteristics in irradiated DNA .
	manualset3
177009	5	413710	7	NULL	NULL	0	NULL	track characteristics	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These measurements of radical density and spatial extent provide the first direct experimental determination of track characteristics in irradiated DNA .
	manualset3
177010	6	413710	7	NULL	NULL	0	NULL	irradiated DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These measurements of radical density and spatial extent provide the first direct experimental determination of track characteristics in irradiated DNA .
	manualset3
177011	1	413711	7	NULL	NULL	0	NULL	measurements	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These measurements were obtained during brief plantar flexion maximum voluntary isometric contractions ( MVICs ) , and normalised by the superimposed maximal M-wave ( EMG/M ( SUP ) and V/M ( SUP ) , respectively ) , before and after ( 20 s , 10 min and 20 min ) a fatigue protocol ( seven 25 s MVICs , 5 s rest ) .
	manualset3
177012	2	413711	7	NULL	NULL	0	NULL	brief plantar flexion maximum voluntary isometric contractions ( MVICs )	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These measurements were obtained during brief plantar flexion maximum voluntary isometric contractions ( MVICs ) , and normalised by the superimposed maximal M-wave ( EMG/M ( SUP ) and V/M ( SUP ) , respectively ) , before and after ( 20 s , 10 min and 20 min ) a fatigue protocol ( seven 25 s MVICs , 5 s rest ) .
	manualset3
177013	3	413711	7	NULL	NULL	NULL	NULL	superimposed maximal M-wave ( EMG/M ( SUP ) and V/M ( SUP )	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These measurements were obtained during brief plantar flexion maximum voluntary isometric contractions ( MVICs ) , and normalised by the superimposed maximal M-wave ( EMG/M ( SUP ) and V/M ( SUP ) , respectively ) , before and after ( 20 s , 10 min and 20 min ) a fatigue protocol ( seven 25 s MVICs , 5 s rest ) .
	manualset3
177014	4	413711	7	NULL	NULL	0	NULL	20 s	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	These measurements were obtained during brief plantar flexion maximum voluntary isometric contractions ( MVICs ) , and normalised by the superimposed maximal M-wave ( EMG/M ( SUP ) and V/M ( SUP ) , respectively ) , before and after ( 20 s , 10 min and 20 min ) a fatigue protocol ( seven 25 s MVICs , 5 s rest ) .
	manualset3
177015	5	413711	7	NULL	NULL	0	NULL	 10 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	These measurements were obtained during brief plantar flexion maximum voluntary isometric contractions ( MVICs ) , and normalised by the superimposed maximal M-wave ( EMG/M ( SUP ) and V/M ( SUP ) , respectively ) , before and after ( 20 s , 10 min and 20 min ) a fatigue protocol ( seven 25 s MVICs , 5 s rest ) .
	manualset3
177016	6	413711	7	NULL	NULL	0	NULL	20 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	These measurements were obtained during brief plantar flexion maximum voluntary isometric contractions ( MVICs ) , and normalised by the superimposed maximal M-wave ( EMG/M ( SUP ) and V/M ( SUP ) , respectively ) , before and after ( 20 s , 10 min and 20 min ) a fatigue protocol ( seven 25 s MVICs , 5 s rest ) .
	manualset3
177017	7	413711	7	NULL	NULL	0	NULL	fatigue protocol	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These measurements were obtained during brief plantar flexion maximum voluntary isometric contractions ( MVICs ) , and normalised by the superimposed maximal M-wave ( EMG/M ( SUP ) and V/M ( SUP ) , respectively ) , before and after ( 20 s , 10 min and 20 min ) a fatigue protocol ( seven 25 s MVICs , 5 s rest ) .
	manualset3
177018	8	413711	7	NULL	NULL	NULL	NULL	seven 25 s MVICs	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These measurements were obtained during brief plantar flexion maximum voluntary isometric contractions ( MVICs ) , and normalised by the superimposed maximal M-wave ( EMG/M ( SUP ) and V/M ( SUP ) , respectively ) , before and after ( 20 s , 10 min and 20 min ) a fatigue protocol ( seven 25 s MVICs , 5 s rest ) .
	manualset3
177019	9	413711	7	NULL	NULL	0	NULL	5 s rest 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These measurements were obtained during brief plantar flexion maximum voluntary isometric contractions ( MVICs ) , and normalised by the superimposed maximal M-wave ( EMG/M ( SUP ) and V/M ( SUP ) , respectively ) , before and after ( 20 s , 10 min and 20 min ) a fatigue protocol ( seven 25 s MVICs , 5 s rest ) .
	manualset3
177020	1	413712	7	NULL	NULL	0	NULL	 mechanically polished Nitinol surfaces	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These mechanically polished Nitinol surfaces are compared with chemically passivated and electrochemically polished Nitinol surfaces and mechanically polished titanium surfaces in phosphate buffered saline solution .
	manualset3
177021	2	413712	7	NULL	NULL	0	NULL	electrochemically polished Nitinol surfaces	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These mechanically polished Nitinol surfaces are compared with chemically passivated and electrochemically polished Nitinol surfaces and mechanically polished titanium surfaces in phosphate buffered saline solution .
	manualset3
177022	3	413712	7	NULL	NULL	0	NULL	mechanically polished titanium surfaces	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These mechanically polished Nitinol surfaces are compared with chemically passivated and electrochemically polished Nitinol surfaces and mechanically polished titanium surfaces in phosphate buffered saline solution .
	manualset3
177023	4	413712	7	NULL	NULL	0	NULL	phosphate buffered saline solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These mechanically polished Nitinol surfaces are compared with chemically passivated and electrochemically polished Nitinol surfaces and mechanically polished titanium surfaces in phosphate buffered saline solution .
	manualset3
177024	1	413713	7	NULL	NULL	0	NULL	mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These mechanisms induce tolerance to antigens that reduces allergic symptoms .
	manualset3
177025	2	413713	7	NULL	NULL	0	NULL	 tolerance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These mechanisms induce tolerance to antigens that reduces allergic symptoms .
	manualset3
177026	3	413713	7	NULL	NULL	0	NULL	antigens	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These mechanisms induce tolerance to antigens that reduces allergic symptoms .
	manualset3
177027	4	413713	7	NULL	NULL	0	NULL	allergic symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These mechanisms induce tolerance to antigens that reduces allergic symptoms .
	manualset3
177028	1	413714	7	NULL	NULL	NULL	NULL	 mechanistic aspects 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These mechanistic aspects of multiple drug binding are addressed here via several spectroscopic probes including ultraviolet-vis difference spectroscopy , protein and ligand fluorescence , and 15N-edited HSQC nuclear magnetic resonance ( NMR ) with 15N-Phe-labeled CYPs .
	manualset3
177029	2	413714	7	NULL	NULL	0	NULL	multiple drug binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These mechanistic aspects of multiple drug binding are addressed here via several spectroscopic probes including ultraviolet-vis difference spectroscopy , protein and ligand fluorescence , and 15N-edited HSQC nuclear magnetic resonance ( NMR ) with 15N-Phe-labeled CYPs .
	manualset3
177030	3	413714	7	NULL	NULL	0	NULL	spectroscopic probes	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These mechanistic aspects of multiple drug binding are addressed here via several spectroscopic probes including ultraviolet-vis difference spectroscopy , protein and ligand fluorescence , and 15N-edited HSQC nuclear magnetic resonance ( NMR ) with 15N-Phe-labeled CYPs .
	manualset3
177031	4	413714	7	NULL	NULL	0	NULL	ultraviolet-vis difference spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These mechanistic aspects of multiple drug binding are addressed here via several spectroscopic probes including ultraviolet-vis difference spectroscopy , protein and ligand fluorescence , and 15N-edited HSQC nuclear magnetic resonance ( NMR ) with 15N-Phe-labeled CYPs .
	manualset3
177032	5	413714	7	NULL	NULL	0	NULL	protein and ligand fluorescence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These mechanistic aspects of multiple drug binding are addressed here via several spectroscopic probes including ultraviolet-vis difference spectroscopy , protein and ligand fluorescence , and 15N-edited HSQC nuclear magnetic resonance ( NMR ) with 15N-Phe-labeled CYPs .
	manualset3
177033	6	413714	7	NULL	NULL	0	NULL	15N-edited HSQC nuclear magnetic resonance ( NMR )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These mechanistic aspects of multiple drug binding are addressed here via several spectroscopic probes including ultraviolet-vis difference spectroscopy , protein and ligand fluorescence , and 15N-edited HSQC nuclear magnetic resonance ( NMR ) with 15N-Phe-labeled CYPs .
	manualset3
177034	7	413714	7	NULL	NULL	0	NULL	15N-Phe-labeled CYPs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These mechanistic aspects of multiple drug binding are addressed here via several spectroscopic probes including ultraviolet-vis difference spectroscopy , protein and ligand fluorescence , and 15N-edited HSQC nuclear magnetic resonance ( NMR ) with 15N-Phe-labeled CYPs .
	manualset3
177035	1	413715	7	NULL	NULL	0	NULL	Addition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of seminal plasma with an apparently normal composition to a sperm population with a high NCD reactivity restored the sperm SDS resistance to normal , i.e. blocked the NCD-response .
	manualset3
177051	2	413715	7	NULL	NULL	0	NULL	seminal plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of seminal plasma with an apparently normal composition to a sperm population with a high NCD reactivity restored the sperm SDS resistance to normal , i.e. blocked the NCD-response .
	manualset3
177052	3	413715	7	NULL	NULL	0	NULL	normal composition 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of seminal plasma with an apparently normal composition to a sperm population with a high NCD reactivity restored the sperm SDS resistance to normal , i.e. blocked the NCD-response .
	manualset3
177086	4	413715	7	NULL	NULL	0	NULL	sperm population	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of seminal plasma with an apparently normal composition to a sperm population with a high NCD reactivity restored the sperm SDS resistance to normal , i.e. blocked the NCD-response .
	manualset3
177087	5	413715	7	NULL	NULL	NULL	NULL	 high NCD reactivity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Addition of seminal plasma with an apparently normal composition to a sperm population with a high NCD reactivity restored the sperm SDS resistance to normal , i.e. blocked the NCD-response .
	manualset3
177088	6	413715	7	NULL	NULL	NULL	NULL	sperm SDS resistance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Addition of seminal plasma with an apparently normal composition to a sperm population with a high NCD reactivity restored the sperm SDS resistance to normal , i.e. blocked the NCD-response .
	manualset3
177089	7	413715	7	NULL	NULL	0	NULL	normal	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of seminal plasma with an apparently normal composition to a sperm population with a high NCD reactivity restored the sperm SDS resistance to normal , i.e. blocked the NCD-response .
	manualset3
177090	8	413715	7	NULL	NULL	0	NULL	NCD-response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of seminal plasma with an apparently normal composition to a sperm population with a high NCD reactivity restored the sperm SDS resistance to normal , i.e. blocked the NCD-response .
	manualset3
177091	1	413716	7	NULL	NULL	0	NULL	metabolic characteristics	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These metabolic characteristics of the polyamines in the rat lens were correlated with the extremely low activities of ornithine decarboxylase and S-adenosylmethionine decarboxylase .
	manualset3
177092	2	413716	7	NULL	NULL	0	NULL	 polyamines	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These metabolic characteristics of the polyamines in the rat lens were correlated with the extremely low activities of ornithine decarboxylase and S-adenosylmethionine decarboxylase .
	manualset3
177093	3	413716	7	NULL	NULL	0	NULL	rat lens	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These metabolic characteristics of the polyamines in the rat lens were correlated with the extremely low activities of ornithine decarboxylase and S-adenosylmethionine decarboxylase .
	manualset3
177094	4	413716	7	NULL	NULL	0	NULL	 low activities 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These metabolic characteristics of the polyamines in the rat lens were correlated with the extremely low activities of ornithine decarboxylase and S-adenosylmethionine decarboxylase .
	manualset3
177095	5	413716	7	NULL	NULL	0	NULL	ornithine decarboxylase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These metabolic characteristics of the polyamines in the rat lens were correlated with the extremely low activities of ornithine decarboxylase and S-adenosylmethionine decarboxylase .
	manualset3
177096	6	413716	7	NULL	NULL	0	NULL	S-adenosylmethionine decarboxylase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These metabolic characteristics of the polyamines in the rat lens were correlated with the extremely low activities of ornithine decarboxylase and S-adenosylmethionine decarboxylase .
	manualset3
177097	1	413717	7	NULL	NULL	NULL	NULL	methods	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These methods allow the detection of autologous graft contamination and the identification of patients at high risk of disease recurrence by means of post-transplant MRD monitoring .
	manualset3
177098	2	413717	7	NULL	NULL	0	NULL	detection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These methods allow the detection of autologous graft contamination and the identification of patients at high risk of disease recurrence by means of post-transplant MRD monitoring .
	manualset3
177099	3	413717	7	NULL	NULL	0	NULL	autologous graft contamination	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These methods allow the detection of autologous graft contamination and the identification of patients at high risk of disease recurrence by means of post-transplant MRD monitoring .
	manualset3
177100	4	413717	7	NULL	NULL	0	NULL	identification	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These methods allow the detection of autologous graft contamination and the identification of patients at high risk of disease recurrence by means of post-transplant MRD monitoring .
	manualset3
177101	5	413717	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These methods allow the detection of autologous graft contamination and the identification of patients at high risk of disease recurrence by means of post-transplant MRD monitoring .
	manualset3
177102	6	413717	7	NULL	NULL	0	NULL	 high risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These methods allow the detection of autologous graft contamination and the identification of patients at high risk of disease recurrence by means of post-transplant MRD monitoring .
	manualset3
177103	7	413717	7	NULL	NULL	NULL	NULL	disease recurrence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These methods allow the detection of autologous graft contamination and the identification of patients at high risk of disease recurrence by means of post-transplant MRD monitoring .
	manualset3
177104	8	413717	7	NULL	NULL	0	NULL	post-transplant MRD monitoring	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These methods allow the detection of autologous graft contamination and the identification of patients at high risk of disease recurrence by means of post-transplant MRD monitoring .
	manualset3
177105	1	413718	7	NULL	NULL	0	NULL	 mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These mice also have circulating rheumatoid factor ( RF ) and develop histological changes in their joints characterized by pannus formation , cartilage and bone erosions .
	manualset3
177106	2	413718	7	NULL	NULL	NULL	NULL	circulating rheumatoid factor ( RF )	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These mice also have circulating rheumatoid factor ( RF ) and develop histological changes in their joints characterized by pannus formation , cartilage and bone erosions .
	manualset3
177107	3	413718	7	NULL	NULL	0	NULL	histological changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These mice also have circulating rheumatoid factor ( RF ) and develop histological changes in their joints characterized by pannus formation , cartilage and bone erosions .
	manualset3
177108	4	413718	7	NULL	NULL	0	NULL	joints	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These mice also have circulating rheumatoid factor ( RF ) and develop histological changes in their joints characterized by pannus formation , cartilage and bone erosions .
	manualset3
177109	5	413718	7	NULL	NULL	NULL	NULL	 pannus formation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These mice also have circulating rheumatoid factor ( RF ) and develop histological changes in their joints characterized by pannus formation , cartilage and bone erosions .
	manualset3
177110	6	413718	7	NULL	NULL	NULL	NULL	cartilage erosions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These mice also have circulating rheumatoid factor ( RF ) and develop histological changes in their joints characterized by pannus formation , cartilage and bone erosions .
	manualset3
177111	7	413718	7	NULL	NULL	0	NULL	bone erosions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These mice also have circulating rheumatoid factor ( RF ) and develop histological changes in their joints characterized by pannus formation , cartilage and bone erosions .
	manualset3
177112	1	413719	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These mice may be useful models of atopic dermatitis ; preparation of the animals is not particularly time consuming , the reproducibility is 100 % , and atopic dermatitis symptoms occur even in a specific pathogen-free environment .
	manualset3
177113	2	413719	7	NULL	NULL	NULL	NULL	models 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These mice may be useful models of atopic dermatitis ; preparation of the animals is not particularly time consuming , the reproducibility is 100 % , and atopic dermatitis symptoms occur even in a specific pathogen-free environment .
	manualset3
177114	3	413719	7	NULL	NULL	0	NULL	atopic dermatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These mice may be useful models of atopic dermatitis ; preparation of the animals is not particularly time consuming , the reproducibility is 100 % , and atopic dermatitis symptoms occur even in a specific pathogen-free environment .
	manualset3
177115	4	413719	7	NULL	NULL	0	NULL	preparation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These mice may be useful models of atopic dermatitis ; preparation of the animals is not particularly time consuming , the reproducibility is 100 % , and atopic dermatitis symptoms occur even in a specific pathogen-free environment .
	manualset3
177116	5	413719	7	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These mice may be useful models of atopic dermatitis ; preparation of the animals is not particularly time consuming , the reproducibility is 100 % , and atopic dermatitis symptoms occur even in a specific pathogen-free environment .
	manualset3
177117	6	413719	7	NULL	NULL	0	NULL	reproducibility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These mice may be useful models of atopic dermatitis ; preparation of the animals is not particularly time consuming , the reproducibility is 100 % , and atopic dermatitis symptoms occur even in a specific pathogen-free environment .
	manualset3
177118	7	413719	7	NULL	NULL	0	NULL	100 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These mice may be useful models of atopic dermatitis ; preparation of the animals is not particularly time consuming , the reproducibility is 100 % , and atopic dermatitis symptoms occur even in a specific pathogen-free environment .
	manualset3
177119	8	413719	7	NULL	NULL	0	NULL	atopic dermatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These mice may be useful models of atopic dermatitis ; preparation of the animals is not particularly time consuming , the reproducibility is 100 % , and atopic dermatitis symptoms occur even in a specific pathogen-free environment .
	manualset3
177120	9	413719	7	NULL	NULL	0	NULL	symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These mice may be useful models of atopic dermatitis ; preparation of the animals is not particularly time consuming , the reproducibility is 100 % , and atopic dermatitis symptoms occur even in a specific pathogen-free environment .
	manualset3
177121	10	413719	7	NULL	NULL	0	NULL	specific pathogen-free environment 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These mice may be useful models of atopic dermatitis ; preparation of the animals is not particularly time consuming , the reproducibility is 100 % , and atopic dermatitis symptoms occur even in a specific pathogen-free environment .
	manualset3
177122	1	413720	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These mice will be useful for noninvasive monitoring of cutaneous nerve fiber degeneration and loss of heat-induced pain perception during diabetes and for the assessment of efficacy of therapeutic treatment of diabetic neuropathy .
	manualset3
177123	2	413720	7	NULL	NULL	0	NULL	noninvasive monitoring	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These mice will be useful for noninvasive monitoring of cutaneous nerve fiber degeneration and loss of heat-induced pain perception during diabetes and for the assessment of efficacy of therapeutic treatment of diabetic neuropathy .
	manualset3
177124	3	413720	7	NULL	NULL	0	NULL	cutaneous nerve fiber degeneration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These mice will be useful for noninvasive monitoring of cutaneous nerve fiber degeneration and loss of heat-induced pain perception during diabetes and for the assessment of efficacy of therapeutic treatment of diabetic neuropathy .
	manualset3
177125	4	413720	7	NULL	NULL	0	NULL	loss 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These mice will be useful for noninvasive monitoring of cutaneous nerve fiber degeneration and loss of heat-induced pain perception during diabetes and for the assessment of efficacy of therapeutic treatment of diabetic neuropathy .
	manualset3
177126	5	413720	7	NULL	NULL	0	NULL	heat-induced pain perception	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These mice will be useful for noninvasive monitoring of cutaneous nerve fiber degeneration and loss of heat-induced pain perception during diabetes and for the assessment of efficacy of therapeutic treatment of diabetic neuropathy .
	manualset3
177127	6	413720	7	NULL	NULL	0	NULL	diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These mice will be useful for noninvasive monitoring of cutaneous nerve fiber degeneration and loss of heat-induced pain perception during diabetes and for the assessment of efficacy of therapeutic treatment of diabetic neuropathy .
	manualset3
177128	7	413720	7	NULL	NULL	0	NULL	 assessment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These mice will be useful for noninvasive monitoring of cutaneous nerve fiber degeneration and loss of heat-induced pain perception during diabetes and for the assessment of efficacy of therapeutic treatment of diabetic neuropathy .
	manualset3
177129	8	413720	7	NULL	NULL	0	NULL	efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These mice will be useful for noninvasive monitoring of cutaneous nerve fiber degeneration and loss of heat-induced pain perception during diabetes and for the assessment of efficacy of therapeutic treatment of diabetic neuropathy .
	manualset3
177130	9	413720	7	NULL	NULL	0	NULL	therapeutic treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These mice will be useful for noninvasive monitoring of cutaneous nerve fiber degeneration and loss of heat-induced pain perception during diabetes and for the assessment of efficacy of therapeutic treatment of diabetic neuropathy .
	manualset3
177131	10	413720	7	NULL	NULL	0	NULL	diabetic neuropathy 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These mice will be useful for noninvasive monitoring of cutaneous nerve fiber degeneration and loss of heat-induced pain perception during diabetes and for the assessment of efficacy of therapeutic treatment of diabetic neuropathy .
	manualset3
177132	1	413721	7	NULL	NULL	0	NULL	Addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of sucrose to an isotonic gradient in an attempt to balance osmotic conditions during density determinations .
	manualset3
177133	2	413721	7	NULL	NULL	0	NULL	sucrose	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of sucrose to an isotonic gradient in an attempt to balance osmotic conditions during density determinations .
	manualset3
177134	3	413721	7	NULL	NULL	0	NULL	 isotonic gradient 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of sucrose to an isotonic gradient in an attempt to balance osmotic conditions during density determinations .
	manualset3
177135	4	413721	7	NULL	NULL	0	NULL	osmotic conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of sucrose to an isotonic gradient in an attempt to balance osmotic conditions during density determinations .
	manualset3
177136	5	413721	7	NULL	NULL	0	NULL	density determinations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of sucrose to an isotonic gradient in an attempt to balance osmotic conditions during density determinations .
	manualset3
190515	6	413721	7	NULL	NULL	0	NULL	 attempt	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of sucrose to an isotonic gradient in an attempt to balance osmotic conditions during density determinations .
	manualset3
177137	1	413722	7	NULL	NULL	0	NULL	models	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These models have been applied to the interpretation of the variation of radiosensitivity with a linear energy transfer ( LET ) of spores of Bacillus subtilis exposed wet and dry , and good fits to the published experimental data were obtained using both models .
	manualset3
177138	2	413722	7	NULL	NULL	NULL	NULL	interpretation 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These models have been applied to the interpretation of the variation of radiosensitivity with a linear energy transfer ( LET ) of spores of Bacillus subtilis exposed wet and dry , and good fits to the published experimental data were obtained using both models .
	manualset3
177139	3	413722	7	NULL	NULL	0	NULL	variation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These models have been applied to the interpretation of the variation of radiosensitivity with a linear energy transfer ( LET ) of spores of Bacillus subtilis exposed wet and dry , and good fits to the published experimental data were obtained using both models .
	manualset3
177140	4	413722	7	NULL	NULL	NULL	NULL	radiosensitivity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These models have been applied to the interpretation of the variation of radiosensitivity with a linear energy transfer ( LET ) of spores of Bacillus subtilis exposed wet and dry , and good fits to the published experimental data were obtained using both models .
	manualset3
177141	5	413722	7	NULL	NULL	0	NULL	linear energy transfer ( LET )	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These models have been applied to the interpretation of the variation of radiosensitivity with a linear energy transfer ( LET ) of spores of Bacillus subtilis exposed wet and dry , and good fits to the published experimental data were obtained using both models .
	manualset3
177142	6	413722	7	NULL	NULL	0	NULL	spores	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These models have been applied to the interpretation of the variation of radiosensitivity with a linear energy transfer ( LET ) of spores of Bacillus subtilis exposed wet and dry , and good fits to the published experimental data were obtained using both models .
	manualset3
177143	7	413722	7	NULL	NULL	0	NULL	Bacillus subtilis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These models have been applied to the interpretation of the variation of radiosensitivity with a linear energy transfer ( LET ) of spores of Bacillus subtilis exposed wet and dry , and good fits to the published experimental data were obtained using both models .
	manualset3
177144	8	413722	7	NULL	NULL	0	NULL	good fits 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These models have been applied to the interpretation of the variation of radiosensitivity with a linear energy transfer ( LET ) of spores of Bacillus subtilis exposed wet and dry , and good fits to the published experimental data were obtained using both models .
	manualset3
177145	9	413722	7	NULL	NULL	0	NULL	 published experimental data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These models have been applied to the interpretation of the variation of radiosensitivity with a linear energy transfer ( LET ) of spores of Bacillus subtilis exposed wet and dry , and good fits to the published experimental data were obtained using both models .
	manualset3
177146	10	413722	7	NULL	NULL	0	NULL	models	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These models have been applied to the interpretation of the variation of radiosensitivity with a linear energy transfer ( LET ) of spores of Bacillus subtilis exposed wet and dry , and good fits to the published experimental data were obtained using both models .
	manualset3
177147	1	413723	7	NULL	NULL	0	NULL	molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	These molecules are known to be important in normal wound healing .
	manualset3
177148	2	413723	7	NULL	NULL	0	NULL	normal wound healing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These molecules are known to be important in normal wound healing .
	manualset3
177149	1	413724	7	NULL	NULL	0	NULL	mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These mutations , which are apparent progression events , enable MM tumors to become less dependent on bone marrow signals that activate NF-kappaB .
	manualset3
177150	2	413724	7	NULL	NULL	NULL	NULL	 progression events	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These mutations , which are apparent progression events , enable MM tumors to become less dependent on bone marrow signals that activate NF-kappaB .
	manualset3
177151	3	413724	7	NULL	NULL	0	NULL	MM tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These mutations , which are apparent progression events , enable MM tumors to become less dependent on bone marrow signals that activate NF-kappaB .
	manualset3
177152	4	413724	7	NULL	NULL	0	NULL	bone marrow signals	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These mutations , which are apparent progression events , enable MM tumors to become less dependent on bone marrow signals that activate NF-kappaB .
	manualset3
177153	5	413724	7	NULL	NULL	0	NULL	NF-kappaB	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These mutations , which are apparent progression events , enable MM tumors to become less dependent on bone marrow signals that activate NF-kappaB .
	manualset3
177154	1	413725	7	NULL	NULL	0	NULL	myf-5 + cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These myf-5 + cells coexpress neuronal and muscle markers in culture .
	manualset3
177155	2	413725	7	NULL	NULL	0	NULL	neuronal markers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These myf-5 + cells coexpress neuronal and muscle markers in culture .
	manualset3
177156	3	413725	7	NULL	NULL	0	NULL	muscle markers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These myf-5 + cells coexpress neuronal and muscle markers in culture .
	manualset3
177157	4	413725	7	NULL	NULL	0	NULL	culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These myf-5 + cells coexpress neuronal and muscle markers in culture .
	manualset3
177158	1	413726	7	NULL	NULL	0	NULL	 n.s.d.p.s	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These n.s.d.p.s displayed a strong voltage-dependent behavior and were detected only at membrane potentials within 5-7 mV of the threshold for spike initiation .
	manualset3
177159	2	413726	7	NULL	NULL	0	NULL	strong voltage-dependent behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These n.s.d.p.s displayed a strong voltage-dependent behavior and were detected only at membrane potentials within 5-7 mV of the threshold for spike initiation .
	manualset3
177160	3	413726	7	NULL	NULL	0	NULL	membrane potentials	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These n.s.d.p.s displayed a strong voltage-dependent behavior and were detected only at membrane potentials within 5-7 mV of the threshold for spike initiation .
	manualset3
177161	4	413726	7	NULL	NULL	0	NULL	5-7 mV	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These n.s.d.p.s displayed a strong voltage-dependent behavior and were detected only at membrane potentials within 5-7 mV of the threshold for spike initiation .
	manualset3
177162	5	413726	7	NULL	NULL	0	NULL	threshold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These n.s.d.p.s displayed a strong voltage-dependent behavior and were detected only at membrane potentials within 5-7 mV of the threshold for spike initiation .
	manualset3
177163	6	413726	7	NULL	NULL	0	NULL	 spike initiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These n.s.d.p.s displayed a strong voltage-dependent behavior and were detected only at membrane potentials within 5-7 mV of the threshold for spike initiation .
	manualset3
177164	1	413727	7	NULL	NULL	0	NULL	 nanostructures	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	These nanostructures have a width of approximately 333-1 , 000 atoms , assuming that the average dimension of an atom is 1.5 A. The size range of the holes is approximately 40-432 nm ( equivalent to a width of approximately 266-2880 atoms ) .
	manualset3
177165	2	413727	7	NULL	NULL	0	NULL	 width	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These nanostructures have a width of approximately 333-1 , 000 atoms , assuming that the average dimension of an atom is 1.5 A. The size range of the holes is approximately 40-432 nm ( equivalent to a width of approximately 266-2880 atoms ) .
	manualset3
177166	3	413727	7	NULL	NULL	0	NULL	333-1 , 000 atoms	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	These nanostructures have a width of approximately 333-1 , 000 atoms , assuming that the average dimension of an atom is 1.5 A. The size range of the holes is approximately 40-432 nm ( equivalent to a width of approximately 266-2880 atoms ) .
	manualset3
177167	4	413727	7	NULL	NULL	0	NULL	dimension	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These nanostructures have a width of approximately 333-1 , 000 atoms , assuming that the average dimension of an atom is 1.5 A. The size range of the holes is approximately 40-432 nm ( equivalent to a width of approximately 266-2880 atoms ) .
	manualset3
177168	5	413727	7	NULL	NULL	0	NULL	atom	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	These nanostructures have a width of approximately 333-1 , 000 atoms , assuming that the average dimension of an atom is 1.5 A. The size range of the holes is approximately 40-432 nm ( equivalent to a width of approximately 266-2880 atoms ) .
	manualset3
177169	6	413727	7	NULL	NULL	0	NULL	1.5 A	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These nanostructures have a width of approximately 333-1 , 000 atoms , assuming that the average dimension of an atom is 1.5 A. The size range of the holes is approximately 40-432 nm ( equivalent to a width of approximately 266-2880 atoms ) .
	manualset3
177170	7	413727	7	NULL	NULL	0	NULL	size range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These nanostructures have a width of approximately 333-1 , 000 atoms , assuming that the average dimension of an atom is 1.5 A. The size range of the holes is approximately 40-432 nm ( equivalent to a width of approximately 266-2880 atoms ) .
	manualset3
177171	8	413727	7	NULL	NULL	0	NULL	holes	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These nanostructures have a width of approximately 333-1 , 000 atoms , assuming that the average dimension of an atom is 1.5 A. The size range of the holes is approximately 40-432 nm ( equivalent to a width of approximately 266-2880 atoms ) .
	manualset3
177172	9	413727	7	NULL	NULL	0	NULL	40-432 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These nanostructures have a width of approximately 333-1 , 000 atoms , assuming that the average dimension of an atom is 1.5 A. The size range of the holes is approximately 40-432 nm ( equivalent to a width of approximately 266-2880 atoms ) .
	manualset3
177173	10	413727	7	NULL	NULL	0	NULL	width	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These nanostructures have a width of approximately 333-1 , 000 atoms , assuming that the average dimension of an atom is 1.5 A. The size range of the holes is approximately 40-432 nm ( equivalent to a width of approximately 266-2880 atoms ) .
	manualset3
177174	11	413727	7	NULL	NULL	0	NULL	266-2880 atoms 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	These nanostructures have a width of approximately 333-1 , 000 atoms , assuming that the average dimension of an atom is 1.5 A. The size range of the holes is approximately 40-432 nm ( equivalent to a width of approximately 266-2880 atoms ) .
	manualset3
177175	1	413728	7	NULL	NULL	0	NULL	Comparative studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative studies on the value of carbon tetrachloride , paraffine oil and aluminum gel as immunologic adjuvants .
	manualset3
177176	2	413728	7	NULL	NULL	0	NULL	 value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative studies on the value of carbon tetrachloride , paraffine oil and aluminum gel as immunologic adjuvants .
	manualset3
177177	3	413728	7	NULL	NULL	0	NULL	carbon tetrachloride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative studies on the value of carbon tetrachloride , paraffine oil and aluminum gel as immunologic adjuvants .
	manualset3
177178	4	413728	7	NULL	NULL	0	NULL	paraffine oil	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative studies on the value of carbon tetrachloride , paraffine oil and aluminum gel as immunologic adjuvants .
	manualset3
177179	5	413728	7	NULL	NULL	0	NULL	aluminum gel 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative studies on the value of carbon tetrachloride , paraffine oil and aluminum gel as immunologic adjuvants .
	manualset3
177180	6	413728	7	NULL	NULL	0	NULL	immunologic adjuvants	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative studies on the value of carbon tetrachloride , paraffine oil and aluminum gel as immunologic adjuvants .
	manualset3
177181	1	413729	7	NULL	NULL	NULL	NULL	Addition	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Addition of the cAMP phosphodiesterase inhibitor , 3-isobutyl-1-methylxanthine ( IBMX ) permitted detection of the novel adenylyl cyclase activity in lysates of an acaA/acgA double mutant .
	manualset3
177182	2	413729	7	NULL	NULL	0	NULL	cAMP phosphodiesterase inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of the cAMP phosphodiesterase inhibitor , 3-isobutyl-1-methylxanthine ( IBMX ) permitted detection of the novel adenylyl cyclase activity in lysates of an acaA/acgA double mutant .
	manualset3
177183	3	413729	7	NULL	NULL	0	NULL	3-isobutyl-1-methylxanthine ( IBMX )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of the cAMP phosphodiesterase inhibitor , 3-isobutyl-1-methylxanthine ( IBMX ) permitted detection of the novel adenylyl cyclase activity in lysates of an acaA/acgA double mutant .
	manualset3
177184	4	413729	7	NULL	NULL	0	NULL	adenylyl cyclase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of the cAMP phosphodiesterase inhibitor , 3-isobutyl-1-methylxanthine ( IBMX ) permitted detection of the novel adenylyl cyclase activity in lysates of an acaA/acgA double mutant .
	manualset3
177185	5	413729	7	NULL	NULL	NULL	NULL	lysates	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Addition of the cAMP phosphodiesterase inhibitor , 3-isobutyl-1-methylxanthine ( IBMX ) permitted detection of the novel adenylyl cyclase activity in lysates of an acaA/acgA double mutant .
	manualset3
177186	6	413729	7	NULL	NULL	NULL	NULL	acaA/acgA double mutant	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Addition of the cAMP phosphodiesterase inhibitor , 3-isobutyl-1-methylxanthine ( IBMX ) permitted detection of the novel adenylyl cyclase activity in lysates of an acaA/acgA double mutant .
	manualset3
178887	7	413729	7	NULL	NULL	0	NULL	detection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of the cAMP phosphodiesterase inhibitor , 3-isobutyl-1-methylxanthine ( IBMX ) permitted detection of the novel adenylyl cyclase activity in lysates of an acaA/acgA double mutant .
	manualset3
177187	1	413730	7	NULL	NULL	0	NULL	nerve fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These nerve fibers were labeled anterogradely with wheat germ agglutinin-horseradish peroxidase or stained immunohistochemically with anti-tyrosine hydroxylase antibody .
	manualset3
177188	2	413730	7	NULL	NULL	0	NULL	wheat germ agglutinin-horseradish peroxidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These nerve fibers were labeled anterogradely with wheat germ agglutinin-horseradish peroxidase or stained immunohistochemically with anti-tyrosine hydroxylase antibody .
	manualset3
177189	3	413730	7	NULL	NULL	0	NULL	anti-tyrosine hydroxylase antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These nerve fibers were labeled anterogradely with wheat germ agglutinin-horseradish peroxidase or stained immunohistochemically with anti-tyrosine hydroxylase antibody .
	manualset3
177245	1	413731	7	NULL	NULL	0	NULL	neurons 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These neurons do not synthesize serotonin but import extracellular serotonin via MOD-5 / SERT .
	manualset3
177246	2	413731	7	NULL	NULL	0	NULL	 serotonin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These neurons do not synthesize serotonin but import extracellular serotonin via MOD-5 / SERT .
	manualset3
177247	3	413731	7	NULL	NULL	0	NULL	 import	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These neurons do not synthesize serotonin but import extracellular serotonin via MOD-5 / SERT .
	manualset3
177248	4	413731	7	NULL	NULL	0	NULL	extracellular serotonin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These neurons do not synthesize serotonin but import extracellular serotonin via MOD-5 / SERT .
	manualset3
177249	5	413731	7	NULL	NULL	0	NULL	MOD-5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These neurons do not synthesize serotonin but import extracellular serotonin via MOD-5 / SERT .
	manualset3
177250	6	413731	7	NULL	NULL	0	NULL	SERT	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These neurons do not synthesize serotonin but import extracellular serotonin via MOD-5 / SERT .
	manualset3
177251	1	413732	7	NULL	NULL	0	NULL	neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These neurons selectively fired action potentials when the frequency of the swept-sine-wave ( ZAP ) current input was near the resonant frequency .
	manualset3
177252	2	413732	7	NULL	NULL	0	NULL	action potentials	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These neurons selectively fired action potentials when the frequency of the swept-sine-wave ( ZAP ) current input was near the resonant frequency .
	manualset3
177253	3	413732	7	NULL	NULL	0	NULL	frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These neurons selectively fired action potentials when the frequency of the swept-sine-wave ( ZAP ) current input was near the resonant frequency .
	manualset3
177254	4	413732	7	NULL	NULL	NULL	NULL	swept-sine-wave ( ZAP ) current	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These neurons selectively fired action potentials when the frequency of the swept-sine-wave ( ZAP ) current input was near the resonant frequency .
	manualset3
177255	5	413732	7	NULL	NULL	0	NULL	resonant frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These neurons selectively fired action potentials when the frequency of the swept-sine-wave ( ZAP ) current input was near the resonant frequency .
	manualset3
177314	1	413733	7	NULL	NULL	0	NULL	neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These neurons underwent differentiation over the perinatal period that was mainly manifested in the increase of their size as well as in the development of the Golgi complex , granular endoplasmic reticulum and the onset of the dense core vesicle production .
	manualset3
177315	2	413733	7	NULL	NULL	0	NULL	differentiation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These neurons underwent differentiation over the perinatal period that was mainly manifested in the increase of their size as well as in the development of the Golgi complex , granular endoplasmic reticulum and the onset of the dense core vesicle production .
	manualset3
177316	3	413733	7	NULL	NULL	0	NULL	perinatal period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	These neurons underwent differentiation over the perinatal period that was mainly manifested in the increase of their size as well as in the development of the Golgi complex , granular endoplasmic reticulum and the onset of the dense core vesicle production .
	manualset3
177317	4	413733	7	NULL	NULL	0	NULL	increase	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These neurons underwent differentiation over the perinatal period that was mainly manifested in the increase of their size as well as in the development of the Golgi complex , granular endoplasmic reticulum and the onset of the dense core vesicle production .
	manualset3
177318	5	413733	7	NULL	NULL	0	NULL	 size 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These neurons underwent differentiation over the perinatal period that was mainly manifested in the increase of their size as well as in the development of the Golgi complex , granular endoplasmic reticulum and the onset of the dense core vesicle production .
	manualset3
177319	6	413733	7	NULL	NULL	0	NULL	 development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These neurons underwent differentiation over the perinatal period that was mainly manifested in the increase of their size as well as in the development of the Golgi complex , granular endoplasmic reticulum and the onset of the dense core vesicle production .
	manualset3
177320	7	413733	7	NULL	NULL	0	NULL	Golgi complex	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These neurons underwent differentiation over the perinatal period that was mainly manifested in the increase of their size as well as in the development of the Golgi complex , granular endoplasmic reticulum and the onset of the dense core vesicle production .
	manualset3
177321	8	413733	7	NULL	NULL	0	NULL	granular endoplasmic reticulum	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These neurons underwent differentiation over the perinatal period that was mainly manifested in the increase of their size as well as in the development of the Golgi complex , granular endoplasmic reticulum and the onset of the dense core vesicle production .
	manualset3
177322	9	413733	7	NULL	NULL	0	NULL	onset	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These neurons underwent differentiation over the perinatal period that was mainly manifested in the increase of their size as well as in the development of the Golgi complex , granular endoplasmic reticulum and the onset of the dense core vesicle production .
	manualset3
177323	10	413733	7	NULL	NULL	0	NULL	dense core vesicle production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These neurons underwent differentiation over the perinatal period that was mainly manifested in the increase of their size as well as in the development of the Golgi complex , granular endoplasmic reticulum and the onset of the dense core vesicle production .
	manualset3
177325	1	413734	7	NULL	NULL	0	NULL	neurophysiological findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These neurophysiological findings parallel those reported in 2 other developmental disorders , developmental dyslexia and Rett syndrome .
	manualset3
177326	2	413734	7	NULL	NULL	0	NULL	developmental disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These neurophysiological findings parallel those reported in 2 other developmental disorders , developmental dyslexia and Rett syndrome .
	manualset3
177327	3	413734	7	NULL	NULL	NULL	NULL	developmental dyslexia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These neurophysiological findings parallel those reported in 2 other developmental disorders , developmental dyslexia and Rett syndrome .
	manualset3
177328	4	413734	7	NULL	NULL	NULL	NULL	Rett syndrome	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These neurophysiological findings parallel those reported in 2 other developmental disorders , developmental dyslexia and Rett syndrome .
	manualset3
177329	5	413734	7	NULL	NULL	0	NULL	2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These neurophysiological findings parallel those reported in 2 other developmental disorders , developmental dyslexia and Rett syndrome .
	manualset3
177333	1	413735	7	NULL	NULL	0	NULL	neurotransmitter systems	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These neurotransmitter systems mediate the reinforcing effects of alcohol .
	manualset3
177334	2	413735	7	NULL	NULL	0	NULL	reinforcing effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These neurotransmitter systems mediate the reinforcing effects of alcohol .
	manualset3
177335	3	413735	7	NULL	NULL	0	NULL	alcohol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These neurotransmitter systems mediate the reinforcing effects of alcohol .
	manualset3
177336	1	413736	7	NULL	NULL	0	NULL	new approaches	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These new approaches are based either on the substitution of affected neurons by homogous neuroblasts that are able to replace them anatomically and functionally ( fetal neural grafts ) , or on the use of neuroprotective proteins ( by gene therapy ) that are able to promote natural defenses of neural cells .
	manualset3
177337	2	413736	7	NULL	NULL	NULL	NULL	substitution	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These new approaches are based either on the substitution of affected neurons by homogous neuroblasts that are able to replace them anatomically and functionally ( fetal neural grafts ) , or on the use of neuroprotective proteins ( by gene therapy ) that are able to promote natural defenses of neural cells .
	manualset3
177338	3	413736	7	NULL	NULL	0	NULL	affected neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These new approaches are based either on the substitution of affected neurons by homogous neuroblasts that are able to replace them anatomically and functionally ( fetal neural grafts ) , or on the use of neuroprotective proteins ( by gene therapy ) that are able to promote natural defenses of neural cells .
	manualset3
177339	4	413736	7	NULL	NULL	0	NULL	homogous neuroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These new approaches are based either on the substitution of affected neurons by homogous neuroblasts that are able to replace them anatomically and functionally ( fetal neural grafts ) , or on the use of neuroprotective proteins ( by gene therapy ) that are able to promote natural defenses of neural cells .
	manualset3
177340	5	413736	7	NULL	NULL	0	NULL	fetal neural grafts 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These new approaches are based either on the substitution of affected neurons by homogous neuroblasts that are able to replace them anatomically and functionally ( fetal neural grafts ) , or on the use of neuroprotective proteins ( by gene therapy ) that are able to promote natural defenses of neural cells .
	manualset3
177341	6	413736	7	NULL	NULL	NULL	NULL	use	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These new approaches are based either on the substitution of affected neurons by homogous neuroblasts that are able to replace them anatomically and functionally ( fetal neural grafts ) , or on the use of neuroprotective proteins ( by gene therapy ) that are able to promote natural defenses of neural cells .
	manualset3
177342	7	413736	7	NULL	NULL	NULL	NULL	neuroprotective proteins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These new approaches are based either on the substitution of affected neurons by homogous neuroblasts that are able to replace them anatomically and functionally ( fetal neural grafts ) , or on the use of neuroprotective proteins ( by gene therapy ) that are able to promote natural defenses of neural cells .
	manualset3
177343	8	413736	7	NULL	NULL	0	NULL	gene therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These new approaches are based either on the substitution of affected neurons by homogous neuroblasts that are able to replace them anatomically and functionally ( fetal neural grafts ) , or on the use of neuroprotective proteins ( by gene therapy ) that are able to promote natural defenses of neural cells .
	manualset3
177344	9	413736	7	NULL	NULL	0	NULL	natural defenses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These new approaches are based either on the substitution of affected neurons by homogous neuroblasts that are able to replace them anatomically and functionally ( fetal neural grafts ) , or on the use of neuroprotective proteins ( by gene therapy ) that are able to promote natural defenses of neural cells .
	manualset3
177345	10	413736	7	NULL	NULL	0	NULL	neural cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These new approaches are based either on the substitution of affected neurons by homogous neuroblasts that are able to replace them anatomically and functionally ( fetal neural grafts ) , or on the use of neuroprotective proteins ( by gene therapy ) that are able to promote natural defenses of neural cells .
	manualset3
177347	1	413737	7	NULL	NULL	NULL	NULL	Addition	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Addition of total serum lipoprotein caused a rapid decline in enzymatic activity in both cell types , with a t1/2 of 2-2 .5 h ; however , the onset of the decline was immediate in the glial cells but delayed 1-1 .5 h in the neuronal cells .
	manualset3
177348	2	413737	7	NULL	NULL	NULL	NULL	total serum lipoprotein	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Addition of total serum lipoprotein caused a rapid decline in enzymatic activity in both cell types , with a t1/2 of 2-2 .5 h ; however , the onset of the decline was immediate in the glial cells but delayed 1-1 .5 h in the neuronal cells .
	manualset3
177349	3	413737	7	NULL	NULL	NULL	NULL	rapid decline	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Addition of total serum lipoprotein caused a rapid decline in enzymatic activity in both cell types , with a t1/2 of 2-2 .5 h ; however , the onset of the decline was immediate in the glial cells but delayed 1-1 .5 h in the neuronal cells .
	manualset3
177350	4	413737	7	NULL	NULL	0	NULL	enzymatic activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of total serum lipoprotein caused a rapid decline in enzymatic activity in both cell types , with a t1/2 of 2-2 .5 h ; however , the onset of the decline was immediate in the glial cells but delayed 1-1 .5 h in the neuronal cells .
	manualset3
177351	5	413737	7	NULL	NULL	0	NULL	cell types	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of total serum lipoprotein caused a rapid decline in enzymatic activity in both cell types , with a t1/2 of 2-2 .5 h ; however , the onset of the decline was immediate in the glial cells but delayed 1-1 .5 h in the neuronal cells .
	manualset3
177352	6	413737	7	NULL	NULL	0	NULL	t1/2	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of total serum lipoprotein caused a rapid decline in enzymatic activity in both cell types , with a t1/2 of 2-2 .5 h ; however , the onset of the decline was immediate in the glial cells but delayed 1-1 .5 h in the neuronal cells .
	manualset3
177353	7	413737	7	NULL	NULL	0	NULL	2-2 .5 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of total serum lipoprotein caused a rapid decline in enzymatic activity in both cell types , with a t1/2 of 2-2 .5 h ; however , the onset of the decline was immediate in the glial cells but delayed 1-1 .5 h in the neuronal cells .
	manualset3
177362	9	413737	7	NULL	NULL	NULL	NULL	onset of the decline	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Addition of total serum lipoprotein caused a rapid decline in enzymatic activity in both cell types , with a t1/2 of 2-2 .5 h ; however , the onset of the decline was immediate in the glial cells but delayed 1-1 .5 h in the neuronal cells .
	manualset3
177364	10	413737	7	NULL	NULL	0	NULL	glial cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of total serum lipoprotein caused a rapid decline in enzymatic activity in both cell types , with a t1/2 of 2-2 .5 h ; however , the onset of the decline was immediate in the glial cells but delayed 1-1 .5 h in the neuronal cells .
	manualset3
177365	11	413737	7	NULL	NULL	0	NULL	1-1 .5 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of total serum lipoprotein caused a rapid decline in enzymatic activity in both cell types , with a t1/2 of 2-2 .5 h ; however , the onset of the decline was immediate in the glial cells but delayed 1-1 .5 h in the neuronal cells .
	manualset3
177367	12	413737	7	NULL	NULL	0	NULL	neuronal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of total serum lipoprotein caused a rapid decline in enzymatic activity in both cell types , with a t1/2 of 2-2 .5 h ; however , the onset of the decline was immediate in the glial cells but delayed 1-1 .5 h in the neuronal cells .
	manualset3
177388	1	413738	7	NULL	NULL	0	NULL	new estriol conjugates 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These new estriol conjugates comprise less than 1 percent of total , estriol , apparently too low to be of diagnostic value in human pregnancy .
	manualset3
177389	2	413738	7	NULL	NULL	0	NULL	1 percent 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These new estriol conjugates comprise less than 1 percent of total , estriol , apparently too low to be of diagnostic value in human pregnancy .
	manualset3
177390	3	413738	7	NULL	NULL	0	NULL	estriol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These new estriol conjugates comprise less than 1 percent of total , estriol , apparently too low to be of diagnostic value in human pregnancy .
	manualset3
177391	4	413738	7	NULL	NULL	0	NULL	low 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These new estriol conjugates comprise less than 1 percent of total , estriol , apparently too low to be of diagnostic value in human pregnancy .
	manualset3
177392	5	413738	7	NULL	NULL	NULL	NULL	diagnostic value	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These new estriol conjugates comprise less than 1 percent of total , estriol , apparently too low to be of diagnostic value in human pregnancy .
	manualset3
177393	6	413738	7	NULL	NULL	0	NULL	human pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These new estriol conjugates comprise less than 1 percent of total , estriol , apparently too low to be of diagnostic value in human pregnancy .
	manualset3
177394	7	413738	7	NULL	NULL	0	NULL	total	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These new estriol conjugates comprise less than 1 percent of total , estriol , apparently too low to be of diagnostic value in human pregnancy .
	manualset3
177399	1	413739	7	NULL	NULL	0	NULL	new forms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These new forms of retinal lesions differ from retinal folds found in the far periphery of the developing retina .
	manualset3
177400	2	413739	7	NULL	NULL	0	NULL	retinal lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These new forms of retinal lesions differ from retinal folds found in the far periphery of the developing retina .
	manualset3
177402	3	413739	7	NULL	NULL	0	NULL	retinal folds	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These new forms of retinal lesions differ from retinal folds found in the far periphery of the developing retina .
	manualset3
177403	4	413739	7	NULL	NULL	0	NULL	far periphery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These new forms of retinal lesions differ from retinal folds found in the far periphery of the developing retina .
	manualset3
177405	5	413739	7	NULL	NULL	0	NULL	developing retina	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These new forms of retinal lesions differ from retinal folds found in the far periphery of the developing retina .
	manualset3
177409	1	413740	7	NULL	NULL	0	NULL	 nonlinear mixed models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These nonlinear mixed models may be used to analyze energy partitioning in animals , to develop prediction equations of MEI , to evaluate individual efficiency for maintenance , and to assess diets regarding the slope of bias in coefficients of maintenance energy requirements .
	manualset3
177410	2	413740	7	NULL	NULL	0	NULL	energy partitioning	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These nonlinear mixed models may be used to analyze energy partitioning in animals , to develop prediction equations of MEI , to evaluate individual efficiency for maintenance , and to assess diets regarding the slope of bias in coefficients of maintenance energy requirements .
	manualset3
177411	3	413740	7	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These nonlinear mixed models may be used to analyze energy partitioning in animals , to develop prediction equations of MEI , to evaluate individual efficiency for maintenance , and to assess diets regarding the slope of bias in coefficients of maintenance energy requirements .
	manualset3
177412	4	413740	7	NULL	NULL	0	NULL	prediction equations	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These nonlinear mixed models may be used to analyze energy partitioning in animals , to develop prediction equations of MEI , to evaluate individual efficiency for maintenance , and to assess diets regarding the slope of bias in coefficients of maintenance energy requirements .
	manualset3
177413	5	413740	7	NULL	NULL	0	NULL	MEI	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These nonlinear mixed models may be used to analyze energy partitioning in animals , to develop prediction equations of MEI , to evaluate individual efficiency for maintenance , and to assess diets regarding the slope of bias in coefficients of maintenance energy requirements .
	manualset3
177414	6	413740	7	NULL	NULL	0	NULL	individual efficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These nonlinear mixed models may be used to analyze energy partitioning in animals , to develop prediction equations of MEI , to evaluate individual efficiency for maintenance , and to assess diets regarding the slope of bias in coefficients of maintenance energy requirements .
	manualset3
177415	7	413740	7	NULL	NULL	0	NULL	maintenance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These nonlinear mixed models may be used to analyze energy partitioning in animals , to develop prediction equations of MEI , to evaluate individual efficiency for maintenance , and to assess diets regarding the slope of bias in coefficients of maintenance energy requirements .
	manualset3
177416	8	413740	7	NULL	NULL	0	NULL	 diets	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	These nonlinear mixed models may be used to analyze energy partitioning in animals , to develop prediction equations of MEI , to evaluate individual efficiency for maintenance , and to assess diets regarding the slope of bias in coefficients of maintenance energy requirements .
	manualset3
177417	9	413740	7	NULL	NULL	NULL	NULL	 slope of bias	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These nonlinear mixed models may be used to analyze energy partitioning in animals , to develop prediction equations of MEI , to evaluate individual efficiency for maintenance , and to assess diets regarding the slope of bias in coefficients of maintenance energy requirements .
	manualset3
177418	10	413740	7	NULL	NULL	0	NULL	coefficients	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These nonlinear mixed models may be used to analyze energy partitioning in animals , to develop prediction equations of MEI , to evaluate individual efficiency for maintenance , and to assess diets regarding the slope of bias in coefficients of maintenance energy requirements .
	manualset3
177419	11	413740	7	NULL	NULL	0	NULL	maintenance energy requirements	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These nonlinear mixed models may be used to analyze energy partitioning in animals , to develop prediction equations of MEI , to evaluate individual efficiency for maintenance , and to assess diets regarding the slope of bias in coefficients of maintenance energy requirements .
	manualset3
177427	1	413741	7	NULL	NULL	0	NULL	novel crown ethers 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These novel crown ethers not only retain the characteristics of their parent crown ethers since they can 1 ) bind cationic guests and 2 ) serve as templates for making mechanically interlocked molecules ( MIMs ) , such as catenanes and rotaxanes , but they also present coordination sites to connect with secondary building units ( SBUs ) in MOFs .
	manualset3
177428	2	413741	7	NULL	NULL	0	NULL	characteristics	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These novel crown ethers not only retain the characteristics of their parent crown ethers since they can 1 ) bind cationic guests and 2 ) serve as templates for making mechanically interlocked molecules ( MIMs ) , such as catenanes and rotaxanes , but they also present coordination sites to connect with secondary building units ( SBUs ) in MOFs .
	manualset3
177429	3	413741	7	NULL	NULL	0	NULL	parent crown ethers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These novel crown ethers not only retain the characteristics of their parent crown ethers since they can 1 ) bind cationic guests and 2 ) serve as templates for making mechanically interlocked molecules ( MIMs ) , such as catenanes and rotaxanes , but they also present coordination sites to connect with secondary building units ( SBUs ) in MOFs .
	manualset3
177432	4	413741	7	NULL	NULL	0	NULL	cationic guests	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These novel crown ethers not only retain the characteristics of their parent crown ethers since they can 1 ) bind cationic guests and 2 ) serve as templates for making mechanically interlocked molecules ( MIMs ) , such as catenanes and rotaxanes , but they also present coordination sites to connect with secondary building units ( SBUs ) in MOFs .
	manualset3
177434	5	413741	7	NULL	NULL	0	NULL	templates 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These novel crown ethers not only retain the characteristics of their parent crown ethers since they can 1 ) bind cationic guests and 2 ) serve as templates for making mechanically interlocked molecules ( MIMs ) , such as catenanes and rotaxanes , but they also present coordination sites to connect with secondary building units ( SBUs ) in MOFs .
	manualset3
177436	6	413741	7	NULL	NULL	0	NULL	mechanically interlocked molecules ( MIMs )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	These novel crown ethers not only retain the characteristics of their parent crown ethers since they can 1 ) bind cationic guests and 2 ) serve as templates for making mechanically interlocked molecules ( MIMs ) , such as catenanes and rotaxanes , but they also present coordination sites to connect with secondary building units ( SBUs ) in MOFs .
	manualset3
177438	7	413741	7	NULL	NULL	0	NULL	catenanes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These novel crown ethers not only retain the characteristics of their parent crown ethers since they can 1 ) bind cationic guests and 2 ) serve as templates for making mechanically interlocked molecules ( MIMs ) , such as catenanes and rotaxanes , but they also present coordination sites to connect with secondary building units ( SBUs ) in MOFs .
	manualset3
177440	8	413741	7	NULL	NULL	0	NULL	 rotaxanes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These novel crown ethers not only retain the characteristics of their parent crown ethers since they can 1 ) bind cationic guests and 2 ) serve as templates for making mechanically interlocked molecules ( MIMs ) , such as catenanes and rotaxanes , but they also present coordination sites to connect with secondary building units ( SBUs ) in MOFs .
	manualset3
177447	9	413741	7	NULL	NULL	0	NULL	coordination sites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These novel crown ethers not only retain the characteristics of their parent crown ethers since they can 1 ) bind cationic guests and 2 ) serve as templates for making mechanically interlocked molecules ( MIMs ) , such as catenanes and rotaxanes , but they also present coordination sites to connect with secondary building units ( SBUs ) in MOFs .
	manualset3
177448	10	413741	7	NULL	NULL	0	NULL	secondary building units ( SBUs )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These novel crown ethers not only retain the characteristics of their parent crown ethers since they can 1 ) bind cationic guests and 2 ) serve as templates for making mechanically interlocked molecules ( MIMs ) , such as catenanes and rotaxanes , but they also present coordination sites to connect with secondary building units ( SBUs ) in MOFs .
	manualset3
177449	11	413741	7	NULL	NULL	0	NULL	MOFs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These novel crown ethers not only retain the characteristics of their parent crown ethers since they can 1 ) bind cationic guests and 2 ) serve as templates for making mechanically interlocked molecules ( MIMs ) , such as catenanes and rotaxanes , but they also present coordination sites to connect with secondary building units ( SBUs ) in MOFs .
	manualset3
177450	1	413742	7	NULL	NULL	0	NULL	observations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations are opposite to those reported for anticipatory postural adjustments under simple reaction time conditions ( a significant change in the timing without major changes in the magnitude ) .
	manualset3
177451	2	413742	7	NULL	NULL	0	NULL	anticipatory postural adjustments 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations are opposite to those reported for anticipatory postural adjustments under simple reaction time conditions ( a significant change in the timing without major changes in the magnitude ) .
	manualset3
177452	3	413742	7	NULL	NULL	0	NULL	reaction time conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations are opposite to those reported for anticipatory postural adjustments under simple reaction time conditions ( a significant change in the timing without major changes in the magnitude ) .
	manualset3
177453	4	413742	7	NULL	NULL	0	NULL	change	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations are opposite to those reported for anticipatory postural adjustments under simple reaction time conditions ( a significant change in the timing without major changes in the magnitude ) .
	manualset3
177454	5	413742	7	NULL	NULL	0	NULL	timing	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations are opposite to those reported for anticipatory postural adjustments under simple reaction time conditions ( a significant change in the timing without major changes in the magnitude ) .
	manualset3
177455	6	413742	7	NULL	NULL	0	NULL	major changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations are opposite to those reported for anticipatory postural adjustments under simple reaction time conditions ( a significant change in the timing without major changes in the magnitude ) .
	manualset3
177456	7	413742	7	NULL	NULL	0	NULL	magnitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations are opposite to those reported for anticipatory postural adjustments under simple reaction time conditions ( a significant change in the timing without major changes in the magnitude ) .
	manualset3
177457	1	413743	7	NULL	NULL	0	NULL	observations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations collectively suggest that Fyn plays critical roles in promoting accelerated MBP expression during myelinogenesis in a MBP isoform-preferential manner , and QKI may act in the same pathway downstream of Fyn for MBP mRNA homeostasis .
	manualset3
177458	2	413743	7	NULL	NULL	0	NULL	Fyn	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations collectively suggest that Fyn plays critical roles in promoting accelerated MBP expression during myelinogenesis in a MBP isoform-preferential manner , and QKI may act in the same pathway downstream of Fyn for MBP mRNA homeostasis .
	manualset3
177459	3	413743	7	NULL	NULL	0	NULL	critical roles	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations collectively suggest that Fyn plays critical roles in promoting accelerated MBP expression during myelinogenesis in a MBP isoform-preferential manner , and QKI may act in the same pathway downstream of Fyn for MBP mRNA homeostasis .
	manualset3
177460	4	413743	7	NULL	NULL	0	NULL	accelerated MBP expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations collectively suggest that Fyn plays critical roles in promoting accelerated MBP expression during myelinogenesis in a MBP isoform-preferential manner , and QKI may act in the same pathway downstream of Fyn for MBP mRNA homeostasis .
	manualset3
177461	5	413743	7	NULL	NULL	NULL	NULL	 myelinogenesis	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These observations collectively suggest that Fyn plays critical roles in promoting accelerated MBP expression during myelinogenesis in a MBP isoform-preferential manner , and QKI may act in the same pathway downstream of Fyn for MBP mRNA homeostasis .
	manualset3
177462	6	413743	7	NULL	NULL	0	NULL	MBP isoform-preferential manner	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations collectively suggest that Fyn plays critical roles in promoting accelerated MBP expression during myelinogenesis in a MBP isoform-preferential manner , and QKI may act in the same pathway downstream of Fyn for MBP mRNA homeostasis .
	manualset3
177463	7	413743	7	NULL	NULL	0	NULL	 QKI	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations collectively suggest that Fyn plays critical roles in promoting accelerated MBP expression during myelinogenesis in a MBP isoform-preferential manner , and QKI may act in the same pathway downstream of Fyn for MBP mRNA homeostasis .
	manualset3
177464	8	413743	7	NULL	NULL	0	NULL	pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations collectively suggest that Fyn plays critical roles in promoting accelerated MBP expression during myelinogenesis in a MBP isoform-preferential manner , and QKI may act in the same pathway downstream of Fyn for MBP mRNA homeostasis .
	manualset3
177465	9	413743	7	NULL	NULL	0	NULL	downstream 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations collectively suggest that Fyn plays critical roles in promoting accelerated MBP expression during myelinogenesis in a MBP isoform-preferential manner , and QKI may act in the same pathway downstream of Fyn for MBP mRNA homeostasis .
	manualset3
177466	10	413743	7	NULL	NULL	0	NULL	Fyn	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations collectively suggest that Fyn plays critical roles in promoting accelerated MBP expression during myelinogenesis in a MBP isoform-preferential manner , and QKI may act in the same pathway downstream of Fyn for MBP mRNA homeostasis .
	manualset3
177467	11	413743	7	NULL	NULL	0	NULL	MBP mRNA homeostasis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations collectively suggest that Fyn plays critical roles in promoting accelerated MBP expression during myelinogenesis in a MBP isoform-preferential manner , and QKI may act in the same pathway downstream of Fyn for MBP mRNA homeostasis .
	manualset3
177468	1	413744	7	NULL	NULL	0	NULL	observations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations demonstrate that exclusion of ribosomes from the axon occurs early in development , about as soon as the axon can be identified .
	manualset3
177469	2	413744	7	NULL	NULL	0	NULL	exclusion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations demonstrate that exclusion of ribosomes from the axon occurs early in development , about as soon as the axon can be identified .
	manualset3
177470	3	413744	7	NULL	NULL	0	NULL	ribosomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations demonstrate that exclusion of ribosomes from the axon occurs early in development , about as soon as the axon can be identified .
	manualset3
177471	4	413744	7	NULL	NULL	0	NULL	axon	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations demonstrate that exclusion of ribosomes from the axon occurs early in development , about as soon as the axon can be identified .
	manualset3
177472	5	413744	7	NULL	NULL	0	NULL	early	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations demonstrate that exclusion of ribosomes from the axon occurs early in development , about as soon as the axon can be identified .
	manualset3
177473	6	413744	7	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations demonstrate that exclusion of ribosomes from the axon occurs early in development , about as soon as the axon can be identified .
	manualset3
177474	7	413744	7	NULL	NULL	0	NULL	axon	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations demonstrate that exclusion of ribosomes from the axon occurs early in development , about as soon as the axon can be identified .
	manualset3
177475	1	413745	7	NULL	NULL	0	NULL	observations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations indicate that the initiation of the secretory response to GnRH is largely independent of calcium entry , whereas the prolongation of gonadotropin secretion is maintained by calcium influx , in part through voltage-sensitive calcium channels .
	manualset3
177476	2	413745	7	NULL	NULL	NULL	NULL	 initiation 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These observations indicate that the initiation of the secretory response to GnRH is largely independent of calcium entry , whereas the prolongation of gonadotropin secretion is maintained by calcium influx , in part through voltage-sensitive calcium channels .
	manualset3
177477	3	413745	7	NULL	NULL	0	NULL	secretory response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations indicate that the initiation of the secretory response to GnRH is largely independent of calcium entry , whereas the prolongation of gonadotropin secretion is maintained by calcium influx , in part through voltage-sensitive calcium channels .
	manualset3
177478	4	413745	7	NULL	NULL	0	NULL	GnRH 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations indicate that the initiation of the secretory response to GnRH is largely independent of calcium entry , whereas the prolongation of gonadotropin secretion is maintained by calcium influx , in part through voltage-sensitive calcium channels .
	manualset3
177479	5	413745	7	NULL	NULL	0	NULL	calcium entry	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations indicate that the initiation of the secretory response to GnRH is largely independent of calcium entry , whereas the prolongation of gonadotropin secretion is maintained by calcium influx , in part through voltage-sensitive calcium channels .
	manualset3
177480	6	413745	7	NULL	NULL	0	NULL	prolongation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations indicate that the initiation of the secretory response to GnRH is largely independent of calcium entry , whereas the prolongation of gonadotropin secretion is maintained by calcium influx , in part through voltage-sensitive calcium channels .
	manualset3
177481	7	413745	7	NULL	NULL	0	NULL	gonadotropin secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations indicate that the initiation of the secretory response to GnRH is largely independent of calcium entry , whereas the prolongation of gonadotropin secretion is maintained by calcium influx , in part through voltage-sensitive calcium channels .
	manualset3
177482	8	413745	7	NULL	NULL	0	NULL	 calcium influx	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations indicate that the initiation of the secretory response to GnRH is largely independent of calcium entry , whereas the prolongation of gonadotropin secretion is maintained by calcium influx , in part through voltage-sensitive calcium channels .
	manualset3
177483	9	413745	7	NULL	NULL	0	NULL	voltage-sensitive calcium channels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations indicate that the initiation of the secretory response to GnRH is largely independent of calcium entry , whereas the prolongation of gonadotropin secretion is maintained by calcium influx , in part through voltage-sensitive calcium channels .
	manualset3
177503	1	413746	7	NULL	NULL	0	NULL	 observations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations led to the hypothesis that the AhR promotes the growth of MB .
	manualset3
177504	2	413746	7	NULL	NULL	NULL	NULL	hypothesis	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These observations led to the hypothesis that the AhR promotes the growth of MB .
	manualset3
177509	3	413746	7	NULL	NULL	0	NULL	 AhR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations led to the hypothesis that the AhR promotes the growth of MB .
	manualset3
177510	4	413746	7	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations led to the hypothesis that the AhR promotes the growth of MB .
	manualset3
177512	5	413746	7	NULL	NULL	0	NULL	MB	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations led to the hypothesis that the AhR promotes the growth of MB .
	manualset3
177515	1	413747	7	NULL	NULL	0	NULL	 observations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations open prospects for further enhancement for the protective properties of S. sonnei specific protective complex , which should be taken into consideration in developing the vaccinal preparation .
	manualset3
177516	3	413747	7	NULL	NULL	NULL	NULL	enhancement	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These observations open prospects for further enhancement for the protective properties of S. sonnei specific protective complex , which should be taken into consideration in developing the vaccinal preparation .
	manualset3
177517	2	413747	7	NULL	NULL	0	NULL	prospects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations open prospects for further enhancement for the protective properties of S. sonnei specific protective complex , which should be taken into consideration in developing the vaccinal preparation .
	manualset3
177520	4	413747	7	NULL	NULL	0	NULL	protective properties	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations open prospects for further enhancement for the protective properties of S. sonnei specific protective complex , which should be taken into consideration in developing the vaccinal preparation .
	manualset3
177525	5	413747	7	NULL	NULL	0	NULL	S. sonnei specific protective complex 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations open prospects for further enhancement for the protective properties of S. sonnei specific protective complex , which should be taken into consideration in developing the vaccinal preparation .
	manualset3
177526	6	413747	7	NULL	NULL	0	NULL	consideration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations open prospects for further enhancement for the protective properties of S. sonnei specific protective complex , which should be taken into consideration in developing the vaccinal preparation .
	manualset3
177527	7	413747	7	NULL	NULL	0	NULL	vaccinal preparation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations open prospects for further enhancement for the protective properties of S. sonnei specific protective complex , which should be taken into consideration in developing the vaccinal preparation .
	manualset3
177528	1	413748	7	NULL	NULL	0	NULL	observations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest a pivotal role of IL-1 in the regulation of PGE economy by trophoblast cells .
	manualset3
177529	2	413748	7	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest a pivotal role of IL-1 in the regulation of PGE economy by trophoblast cells .
	manualset3
177531	3	413748	7	NULL	NULL	0	NULL	IL-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest a pivotal role of IL-1 in the regulation of PGE economy by trophoblast cells .
	manualset3
177533	4	413748	7	NULL	NULL	0	NULL	regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest a pivotal role of IL-1 in the regulation of PGE economy by trophoblast cells .
	manualset3
177534	5	413748	7	NULL	NULL	0	NULL	PGE 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest a pivotal role of IL-1 in the regulation of PGE economy by trophoblast cells .
	manualset3
177535	6	413748	7	NULL	NULL	0	NULL	 trophoblast cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest a pivotal role of IL-1 in the regulation of PGE economy by trophoblast cells .
	manualset3
177546	1	413749	7	NULL	NULL	0	NULL	observations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that Tyro3 RTKs play roles collaboratively in vaginal development , and Mer is more critical , Axl and Tyro3 support the function of Mer .
	manualset3
177547	2	413749	7	NULL	NULL	0	NULL	Tyro3 RTKs	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that Tyro3 RTKs play roles collaboratively in vaginal development , and Mer is more critical , Axl and Tyro3 support the function of Mer .
	manualset3
177548	3	413749	7	NULL	NULL	0	NULL	vaginal development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that Tyro3 RTKs play roles collaboratively in vaginal development , and Mer is more critical , Axl and Tyro3 support the function of Mer .
	manualset3
177549	4	413749	7	NULL	NULL	0	NULL	Mer	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that Tyro3 RTKs play roles collaboratively in vaginal development , and Mer is more critical , Axl and Tyro3 support the function of Mer .
	manualset3
177550	5	413749	7	NULL	NULL	0	NULL	Axl	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that Tyro3 RTKs play roles collaboratively in vaginal development , and Mer is more critical , Axl and Tyro3 support the function of Mer .
	manualset3
177551	6	413749	7	NULL	NULL	0	NULL	Tyro3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that Tyro3 RTKs play roles collaboratively in vaginal development , and Mer is more critical , Axl and Tyro3 support the function of Mer .
	manualset3
177552	7	413749	7	NULL	NULL	0	NULL	function 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that Tyro3 RTKs play roles collaboratively in vaginal development , and Mer is more critical , Axl and Tyro3 support the function of Mer .
	manualset3
177553	8	413749	7	NULL	NULL	0	NULL	Mer	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that Tyro3 RTKs play roles collaboratively in vaginal development , and Mer is more critical , Axl and Tyro3 support the function of Mer .
	manualset3
177554	1	413750	7	NULL	NULL	0	NULL	observations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that a primary role of the SWI/SNF complex is to promote activator binding to nucleosomal DNA .
	manualset3
177555	2	413750	7	NULL	NULL	0	NULL	 primary role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that a primary role of the SWI/SNF complex is to promote activator binding to nucleosomal DNA .
	manualset3
177556	3	413750	7	NULL	NULL	0	NULL	SWI/SNF complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that a primary role of the SWI/SNF complex is to promote activator binding to nucleosomal DNA .
	manualset3
177557	4	413750	7	NULL	NULL	0	NULL	activator binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that a primary role of the SWI/SNF complex is to promote activator binding to nucleosomal DNA .
	manualset3
177558	5	413750	7	NULL	NULL	0	NULL	nucleosomal DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that a primary role of the SWI/SNF complex is to promote activator binding to nucleosomal DNA .
	manualset3
177559	1	413751	7	NULL	NULL	0	NULL	observations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that despite high levels of P-glycoprotein in MDR cells , a sufficient amount of taxol remains intracellular to accelerate the cell cycle machinery and activate the MAPK pathway .
	manualset3
177560	2	413751	7	NULL	NULL	0	NULL	 high levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that despite high levels of P-glycoprotein in MDR cells , a sufficient amount of taxol remains intracellular to accelerate the cell cycle machinery and activate the MAPK pathway .
	manualset3
177561	3	413751	7	NULL	NULL	0	NULL	P-glycoprotein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that despite high levels of P-glycoprotein in MDR cells , a sufficient amount of taxol remains intracellular to accelerate the cell cycle machinery and activate the MAPK pathway .
	manualset3
177562	4	413751	7	NULL	NULL	0	NULL	MDR cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that despite high levels of P-glycoprotein in MDR cells , a sufficient amount of taxol remains intracellular to accelerate the cell cycle machinery and activate the MAPK pathway .
	manualset3
177563	5	413751	7	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that despite high levels of P-glycoprotein in MDR cells , a sufficient amount of taxol remains intracellular to accelerate the cell cycle machinery and activate the MAPK pathway .
	manualset3
177564	6	413751	7	NULL	NULL	0	NULL	taxol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that despite high levels of P-glycoprotein in MDR cells , a sufficient amount of taxol remains intracellular to accelerate the cell cycle machinery and activate the MAPK pathway .
	manualset3
177566	8	413751	7	NULL	NULL	0	NULL	cell cycle machinery	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that despite high levels of P-glycoprotein in MDR cells , a sufficient amount of taxol remains intracellular to accelerate the cell cycle machinery and activate the MAPK pathway .
	manualset3
177567	9	413751	7	NULL	NULL	0	NULL	MAPK pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that despite high levels of P-glycoprotein in MDR cells , a sufficient amount of taxol remains intracellular to accelerate the cell cycle machinery and activate the MAPK pathway .
	manualset3
177568	1	413752	7	NULL	NULL	0	NULL	observations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that sequences in the signal anchor region and stem region allow the Golgi apparatus localization of the membrane-bound and soluble forms of the sialytransferase , respectively , and that both regions may contain Golgi apparatus localization signals .
	manualset3
177569	2	413752	7	NULL	NULL	0	NULL	sequences	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that sequences in the signal anchor region and stem region allow the Golgi apparatus localization of the membrane-bound and soluble forms of the sialytransferase , respectively , and that both regions may contain Golgi apparatus localization signals .
	manualset3
177570	3	413752	7	NULL	NULL	0	NULL	signal anchor region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that sequences in the signal anchor region and stem region allow the Golgi apparatus localization of the membrane-bound and soluble forms of the sialytransferase , respectively , and that both regions may contain Golgi apparatus localization signals .
	manualset3
177571	4	413752	7	NULL	NULL	0	NULL	stem region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that sequences in the signal anchor region and stem region allow the Golgi apparatus localization of the membrane-bound and soluble forms of the sialytransferase , respectively , and that both regions may contain Golgi apparatus localization signals .
	manualset3
177572	5	413752	7	NULL	NULL	0	NULL	Golgi apparatus localization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that sequences in the signal anchor region and stem region allow the Golgi apparatus localization of the membrane-bound and soluble forms of the sialytransferase , respectively , and that both regions may contain Golgi apparatus localization signals .
	manualset3
177573	6	413752	7	NULL	NULL	0	NULL	membrane-bound form of sialytransferase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that sequences in the signal anchor region and stem region allow the Golgi apparatus localization of the membrane-bound and soluble forms of the sialytransferase , respectively , and that both regions may contain Golgi apparatus localization signals .
	manualset3
177574	7	413752	7	NULL	NULL	0	NULL	soluble forms of the sialytransferase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that sequences in the signal anchor region and stem region allow the Golgi apparatus localization of the membrane-bound and soluble forms of the sialytransferase , respectively , and that both regions may contain Golgi apparatus localization signals .
	manualset3
177575	8	413752	7	NULL	NULL	0	NULL	regions	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that sequences in the signal anchor region and stem region allow the Golgi apparatus localization of the membrane-bound and soluble forms of the sialytransferase , respectively , and that both regions may contain Golgi apparatus localization signals .
	manualset3
177576	9	413752	7	NULL	NULL	0	NULL	Golgi apparatus localization signals	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that sequences in the signal anchor region and stem region allow the Golgi apparatus localization of the membrane-bound and soluble forms of the sialytransferase , respectively , and that both regions may contain Golgi apparatus localization signals .
	manualset3
177577	1	413753	7	NULL	NULL	0	NULL	observations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that the mutation in the torsinA protein responsible for DYT1 dystonia may interfere with transport or release of DA , but does not alter pre-synaptic transporters or post-synaptic DA receptors .
	manualset3
177578	2	413753	7	NULL	NULL	0	NULL	mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that the mutation in the torsinA protein responsible for DYT1 dystonia may interfere with transport or release of DA , but does not alter pre-synaptic transporters or post-synaptic DA receptors .
	manualset3
177579	3	413753	7	NULL	NULL	0	NULL	torsinA protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that the mutation in the torsinA protein responsible for DYT1 dystonia may interfere with transport or release of DA , but does not alter pre-synaptic transporters or post-synaptic DA receptors .
	manualset3
177580	4	413753	7	NULL	NULL	0	NULL	DYT1 dystonia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that the mutation in the torsinA protein responsible for DYT1 dystonia may interfere with transport or release of DA , but does not alter pre-synaptic transporters or post-synaptic DA receptors .
	manualset3
177581	5	413753	7	NULL	NULL	0	NULL	transport	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that the mutation in the torsinA protein responsible for DYT1 dystonia may interfere with transport or release of DA , but does not alter pre-synaptic transporters or post-synaptic DA receptors .
	manualset3
177582	6	413753	7	NULL	NULL	0	NULL	release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that the mutation in the torsinA protein responsible for DYT1 dystonia may interfere with transport or release of DA , but does not alter pre-synaptic transporters or post-synaptic DA receptors .
	manualset3
177583	7	413753	7	NULL	NULL	0	NULL	DA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that the mutation in the torsinA protein responsible for DYT1 dystonia may interfere with transport or release of DA , but does not alter pre-synaptic transporters or post-synaptic DA receptors .
	manualset3
177584	8	413753	7	NULL	NULL	0	NULL	pre-synaptic transporters 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that the mutation in the torsinA protein responsible for DYT1 dystonia may interfere with transport or release of DA , but does not alter pre-synaptic transporters or post-synaptic DA receptors .
	manualset3
177585	9	413753	7	NULL	NULL	0	NULL	 post-synaptic DA receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations suggest that the mutation in the torsinA protein responsible for DYT1 dystonia may interfere with transport or release of DA , but does not alter pre-synaptic transporters or post-synaptic DA receptors .
	manualset3
177586	1	413754	7	NULL	NULL	0	NULL	observations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations support a new view that FDCs belong to the reticular cell population .
	manualset3
177587	2	413754	7	NULL	NULL	0	NULL	new view	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations support a new view that FDCs belong to the reticular cell population .
	manualset3
177588	3	413754	7	NULL	NULL	0	NULL	FDCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations support a new view that FDCs belong to the reticular cell population .
	manualset3
177589	4	413754	7	NULL	NULL	0	NULL	reticular cell population	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations support a new view that FDCs belong to the reticular cell population .
	manualset3
177590	1	413755	7	NULL	NULL	0	NULL	biochemical findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These opposing biochemical findings suggest physiologic changes associated with differences in hydration status , likely attributed to different dietary and hydration strategies used by the respective kennels .
	manualset3
177591	2	413755	7	NULL	NULL	0	NULL	physiologic changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These opposing biochemical findings suggest physiologic changes associated with differences in hydration status , likely attributed to different dietary and hydration strategies used by the respective kennels .
	manualset3
177592	3	413755	7	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These opposing biochemical findings suggest physiologic changes associated with differences in hydration status , likely attributed to different dietary and hydration strategies used by the respective kennels .
	manualset3
177593	4	413755	7	NULL	NULL	0	NULL	hydration status	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These opposing biochemical findings suggest physiologic changes associated with differences in hydration status , likely attributed to different dietary and hydration strategies used by the respective kennels .
	manualset3
177594	5	413755	7	NULL	NULL	NULL	NULL	 dietary strategies	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These opposing biochemical findings suggest physiologic changes associated with differences in hydration status , likely attributed to different dietary and hydration strategies used by the respective kennels .
	manualset3
177595	6	413755	7	NULL	NULL	0	NULL	hydration strategies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These opposing biochemical findings suggest physiologic changes associated with differences in hydration status , likely attributed to different dietary and hydration strategies used by the respective kennels .
	manualset3
177596	7	413755	7	NULL	NULL	NULL	NULL	kennels	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These opposing biochemical findings suggest physiologic changes associated with differences in hydration status , likely attributed to different dietary and hydration strategies used by the respective kennels .
	manualset3
177659	1	413756	7	NULL	NULL	0	NULL	organisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These organisms recently have shown a dramatic increase in antibiotic resistance .
	manualset3
177660	2	413756	7	NULL	NULL	NULL	NULL	increase	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These organisms recently have shown a dramatic increase in antibiotic resistance .
	manualset3
177661	3	413756	7	NULL	NULL	NULL	NULL	antibiotic resistance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These organisms recently have shown a dramatic increase in antibiotic resistance .
	manualset3
177662	1	413757	7	NULL	NULL	0	NULL	EGFR-targeting agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional EGFR-targeting agents in clinical development for SCCHN include other EGFR-directed antibodies , tyrosine kinase inhibitors and antisense DNA .
	manualset3
177663	2	413757	7	NULL	NULL	0	NULL	clinical development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional EGFR-targeting agents in clinical development for SCCHN include other EGFR-directed antibodies , tyrosine kinase inhibitors and antisense DNA .
	manualset3
177664	3	413757	7	NULL	NULL	0	NULL	SCCHN	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional EGFR-targeting agents in clinical development for SCCHN include other EGFR-directed antibodies , tyrosine kinase inhibitors and antisense DNA .
	manualset3
177665	4	413757	7	NULL	NULL	0	NULL	EGFR-directed antibodies	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional EGFR-targeting agents in clinical development for SCCHN include other EGFR-directed antibodies , tyrosine kinase inhibitors and antisense DNA .
	manualset3
177666	5	413757	7	NULL	NULL	0	NULL	 tyrosine kinase inhibitors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional EGFR-targeting agents in clinical development for SCCHN include other EGFR-directed antibodies , tyrosine kinase inhibitors and antisense DNA .
	manualset3
177667	6	413757	7	NULL	NULL	0	NULL	antisense DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional EGFR-targeting agents in clinical development for SCCHN include other EGFR-directed antibodies , tyrosine kinase inhibitors and antisense DNA .
	manualset3
177668	1	413758	7	NULL	NULL	0	NULL	oxotungsten ( V ) complexes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These oxotungsten ( V ) complexes display lower reduction potentials than their molybdenum counterparts , underscoring the preference of tungsten for higher oxidation states .
	manualset3
177669	2	413758	7	NULL	NULL	0	NULL	reduction potentials	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These oxotungsten ( V ) complexes display lower reduction potentials than their molybdenum counterparts , underscoring the preference of tungsten for higher oxidation states .
	manualset3
177670	3	413758	7	NULL	NULL	0	NULL	molybdenum counterparts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These oxotungsten ( V ) complexes display lower reduction potentials than their molybdenum counterparts , underscoring the preference of tungsten for higher oxidation states .
	manualset3
177672	5	413758	7	NULL	NULL	0	NULL	tungsten	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These oxotungsten ( V ) complexes display lower reduction potentials than their molybdenum counterparts , underscoring the preference of tungsten for higher oxidation states .
	manualset3
177673	6	413758	7	NULL	NULL	0	NULL	 higher oxidation states	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These oxotungsten ( V ) complexes display lower reduction potentials than their molybdenum counterparts , underscoring the preference of tungsten for higher oxidation states .
	manualset3
177674	1	413759	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These patients suffered from high pressure chronic retention , a syndrome characterized by impairment of renal function and hypertension .
	manualset3
177675	2	413759	7	NULL	NULL	0	NULL	 high pressure chronic retention	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These patients suffered from high pressure chronic retention , a syndrome characterized by impairment of renal function and hypertension .
	manualset3
177676	3	413759	7	NULL	NULL	0	NULL	syndrome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These patients suffered from high pressure chronic retention , a syndrome characterized by impairment of renal function and hypertension .
	manualset3
177677	4	413759	7	NULL	NULL	0	NULL	impairment 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These patients suffered from high pressure chronic retention , a syndrome characterized by impairment of renal function and hypertension .
	manualset3
177678	5	413759	7	NULL	NULL	0	NULL	renal function 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These patients suffered from high pressure chronic retention , a syndrome characterized by impairment of renal function and hypertension .
	manualset3
177679	6	413759	7	NULL	NULL	0	NULL	hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These patients suffered from high pressure chronic retention , a syndrome characterized by impairment of renal function and hypertension .
	manualset3
177680	1	413760	7	NULL	NULL	0	NULL	patterns	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These patterns were seen both in the wind tunnel and in the field .
	manualset3
177719	2	413760	7	NULL	NULL	0	NULL	wind tunnel	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	These patterns were seen both in the wind tunnel and in the field .
	manualset3
177720	3	413760	7	NULL	NULL	0	NULL	field 	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	These patterns were seen both in the wind tunnel and in the field .
	manualset3
177721	1	413761	7	NULL	NULL	0	NULL	peaks 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These peaks are shown to correspond to differently charged forms of MLCK with the charge difference between alpha and beta twice as large as between beta and gamma .
	manualset3
177722	2	413761	7	NULL	NULL	0	NULL	differently charged forms	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These peaks are shown to correspond to differently charged forms of MLCK with the charge difference between alpha and beta twice as large as between beta and gamma .
	manualset3
177723	3	413761	7	NULL	NULL	0	NULL	MLCK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These peaks are shown to correspond to differently charged forms of MLCK with the charge difference between alpha and beta twice as large as between beta and gamma .
	manualset3
177724	4	413761	7	NULL	NULL	0	NULL	charge difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These peaks are shown to correspond to differently charged forms of MLCK with the charge difference between alpha and beta twice as large as between beta and gamma .
	manualset3
177725	5	413761	7	NULL	NULL	0	NULL	alpha	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These peaks are shown to correspond to differently charged forms of MLCK with the charge difference between alpha and beta twice as large as between beta and gamma .
	manualset3
177726	6	413761	7	NULL	NULL	0	NULL	beta	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These peaks are shown to correspond to differently charged forms of MLCK with the charge difference between alpha and beta twice as large as between beta and gamma .
	manualset3
177727	7	413761	7	NULL	NULL	0	NULL	twice	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These peaks are shown to correspond to differently charged forms of MLCK with the charge difference between alpha and beta twice as large as between beta and gamma .
	manualset3
177730	9	413761	7	NULL	NULL	0	NULL	beta	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These peaks are shown to correspond to differently charged forms of MLCK with the charge difference between alpha and beta twice as large as between beta and gamma .
	manualset3
177732	10	413761	7	NULL	NULL	0	NULL	gamma	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These peaks are shown to correspond to differently charged forms of MLCK with the charge difference between alpha and beta twice as large as between beta and gamma .
	manualset3
177744	1	413762	7	NULL	NULL	0	NULL	 peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	These peptides can then be used in affinity chromatography to increase the specificity of polyclonal sera .
	manualset3
177745	2	413762	7	NULL	NULL	0	NULL	affinity chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These peptides can then be used in affinity chromatography to increase the specificity of polyclonal sera .
	manualset3
177746	3	413762	7	NULL	NULL	NULL	NULL	specificity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These peptides can then be used in affinity chromatography to increase the specificity of polyclonal sera .
	manualset3
177747	4	413762	7	NULL	NULL	0	NULL	polyclonal sera	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These peptides can then be used in affinity chromatography to increase the specificity of polyclonal sera .
	manualset3
177748	1	413763	7	NULL	NULL	0	NULL	phosphorylated intermediates	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These phosphorylated intermediates at the stress-activated pathway induce expression of matrix metalloproteinases ( MMPs ) , leading to inflammatory responses and pathological damages involved in the etiology of multiple sclerosis ( MS ) .
	manualset3
177749	2	413763	7	NULL	NULL	0	NULL	stress-activated pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These phosphorylated intermediates at the stress-activated pathway induce expression of matrix metalloproteinases ( MMPs ) , leading to inflammatory responses and pathological damages involved in the etiology of multiple sclerosis ( MS ) .
	manualset3
177750	3	413763	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These phosphorylated intermediates at the stress-activated pathway induce expression of matrix metalloproteinases ( MMPs ) , leading to inflammatory responses and pathological damages involved in the etiology of multiple sclerosis ( MS ) .
	manualset3
177751	4	413763	7	NULL	NULL	0	NULL	matrix metalloproteinases ( MMPs )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These phosphorylated intermediates at the stress-activated pathway induce expression of matrix metalloproteinases ( MMPs ) , leading to inflammatory responses and pathological damages involved in the etiology of multiple sclerosis ( MS ) .
	manualset3
177752	5	413763	7	NULL	NULL	0	NULL	inflammatory responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These phosphorylated intermediates at the stress-activated pathway induce expression of matrix metalloproteinases ( MMPs ) , leading to inflammatory responses and pathological damages involved in the etiology of multiple sclerosis ( MS ) .
	manualset3
177753	6	413763	7	NULL	NULL	0	NULL	pathological damages 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These phosphorylated intermediates at the stress-activated pathway induce expression of matrix metalloproteinases ( MMPs ) , leading to inflammatory responses and pathological damages involved in the etiology of multiple sclerosis ( MS ) .
	manualset3
177754	7	413763	7	NULL	NULL	0	NULL	 etiology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These phosphorylated intermediates at the stress-activated pathway induce expression of matrix metalloproteinases ( MMPs ) , leading to inflammatory responses and pathological damages involved in the etiology of multiple sclerosis ( MS ) .
	manualset3
177755	8	413763	7	NULL	NULL	0	NULL	multiple sclerosis ( MS )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These phosphorylated intermediates at the stress-activated pathway induce expression of matrix metalloproteinases ( MMPs ) , leading to inflammatory responses and pathological damages involved in the etiology of multiple sclerosis ( MS ) .
	manualset3
177761	1	413764	7	NULL	NULL	0	NULL	pigments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These pigments were isolated , purified , and identified by LSI-MS and NMR ( ( 1 ) H , DQF-COSY , ROESY , HSQC , and HMBC ) techniques .
	manualset3
177763	2	413764	7	NULL	NULL	NULL	NULL	LSI-MS technique	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These pigments were isolated , purified , and identified by LSI-MS and NMR ( ( 1 ) H , DQF-COSY , ROESY , HSQC , and HMBC ) techniques .
	manualset3
177765	3	413764	7	NULL	NULL	NULL	NULL	 NMR ( ( 1 ) H technique	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These pigments were isolated , purified , and identified by LSI-MS and NMR ( ( 1 ) H , DQF-COSY , ROESY , HSQC , and HMBC ) techniques .
	manualset3
177767	4	413764	7	NULL	NULL	0	NULL	DQF-COSY technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These pigments were isolated , purified , and identified by LSI-MS and NMR ( ( 1 ) H , DQF-COSY , ROESY , HSQC , and HMBC ) techniques .
	manualset3
177769	5	413764	7	NULL	NULL	0	NULL	ROESY technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These pigments were isolated , purified , and identified by LSI-MS and NMR ( ( 1 ) H , DQF-COSY , ROESY , HSQC , and HMBC ) techniques .
	manualset3
177771	6	413764	7	NULL	NULL	0	NULL	HSQC technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These pigments were isolated , purified , and identified by LSI-MS and NMR ( ( 1 ) H , DQF-COSY , ROESY , HSQC , and HMBC ) techniques .
	manualset3
177772	7	413764	7	NULL	NULL	0	NULL	HMBC technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These pigments were isolated , purified , and identified by LSI-MS and NMR ( ( 1 ) H , DQF-COSY , ROESY , HSQC , and HMBC ) techniques .
	manualset3
177776	1	413765	7	NULL	NULL	0	NULL	 plaque assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These plaque assays are generally very tedious and labor intensive and have modest throughput and high associated variability .
	manualset3
177780	2	413765	7	NULL	NULL	0	NULL	labor intensive	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These plaque assays are generally very tedious and labor intensive and have modest throughput and high associated variability .
	manualset3
177781	4	413765	7	NULL	NULL	NULL	NULL	high associated variability	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These plaque assays are generally very tedious and labor intensive and have modest throughput and high associated variability .
	manualset3
177782	3	413765	7	NULL	NULL	0	NULL	modest throughput	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These plaque assays are generally very tedious and labor intensive and have modest throughput and high associated variability .
	manualset3
177783	1	413766	7	NULL	NULL	NULL	NULL	polymorphisms	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These polymorphisms , occurring in a single form or in connection with other polymorphisms , seem to be implicated in Pb-induced hypertension , e.g. , vitamin D receptor gene .
	manualset3
177784	2	413766	7	NULL	NULL	NULL	NULL	single form	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These polymorphisms , occurring in a single form or in connection with other polymorphisms , seem to be implicated in Pb-induced hypertension , e.g. , vitamin D receptor gene .
	manualset3
177785	3	413766	7	NULL	NULL	0	NULL	connection	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These polymorphisms , occurring in a single form or in connection with other polymorphisms , seem to be implicated in Pb-induced hypertension , e.g. , vitamin D receptor gene .
	manualset3
177786	4	413766	7	NULL	NULL	NULL	NULL	polymorphisms	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These polymorphisms , occurring in a single form or in connection with other polymorphisms , seem to be implicated in Pb-induced hypertension , e.g. , vitamin D receptor gene .
	manualset3
177787	5	413766	7	NULL	NULL	0	NULL	Pb-induced hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These polymorphisms , occurring in a single form or in connection with other polymorphisms , seem to be implicated in Pb-induced hypertension , e.g. , vitamin D receptor gene .
	manualset3
177788	6	413766	7	NULL	NULL	0	NULL	vitamin D receptor gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	These polymorphisms , occurring in a single form or in connection with other polymorphisms , seem to be implicated in Pb-induced hypertension , e.g. , vitamin D receptor gene .
	manualset3
177789	1	413767	7	NULL	NULL	NULL	NULL	polymorphisms	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These polymorphisms subdivide the common allelic variant of C2 ( C2C ) and reveal that there is much greater variability at the C2 locus than that detected by protein typing .
	manualset3
177790	2	413767	7	NULL	NULL	0	NULL	common allelic variant	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	These polymorphisms subdivide the common allelic variant of C2 ( C2C ) and reveal that there is much greater variability at the C2 locus than that detected by protein typing .
	manualset3
177791	3	413767	7	NULL	NULL	0	NULL	C2 ( C2C )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	These polymorphisms subdivide the common allelic variant of C2 ( C2C ) and reveal that there is much greater variability at the C2 locus than that detected by protein typing .
	manualset3
177792	4	413767	7	NULL	NULL	0	NULL	variability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These polymorphisms subdivide the common allelic variant of C2 ( C2C ) and reveal that there is much greater variability at the C2 locus than that detected by protein typing .
	manualset3
177793	5	413767	7	NULL	NULL	0	NULL	C2 locus	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	These polymorphisms subdivide the common allelic variant of C2 ( C2C ) and reveal that there is much greater variability at the C2 locus than that detected by protein typing .
	manualset3
177794	6	413767	7	NULL	NULL	0	NULL	protein typing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These polymorphisms subdivide the common allelic variant of C2 ( C2C ) and reveal that there is much greater variability at the C2 locus than that detected by protein typing .
	manualset3
177795	1	413768	7	NULL	NULL	0	NULL	polypeptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	These polypeptides containing repetitive RGD sequences were able to inhibit experimental and spontaneous lung metastases of B16-BL6 cells more effectively than the corresponding monomer peptides .
	manualset3
177796	2	413768	7	NULL	NULL	0	NULL	repetitive RGD sequences	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	These polypeptides containing repetitive RGD sequences were able to inhibit experimental and spontaneous lung metastases of B16-BL6 cells more effectively than the corresponding monomer peptides .
	manualset3
177797	3	413768	7	NULL	NULL	0	NULL	experimental and spontaneous lung metastases	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These polypeptides containing repetitive RGD sequences were able to inhibit experimental and spontaneous lung metastases of B16-BL6 cells more effectively than the corresponding monomer peptides .
	manualset3
177798	4	413768	7	NULL	NULL	0	NULL	B16-BL6 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These polypeptides containing repetitive RGD sequences were able to inhibit experimental and spontaneous lung metastases of B16-BL6 cells more effectively than the corresponding monomer peptides .
	manualset3
177799	5	413768	7	NULL	NULL	0	NULL	monomer peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	These polypeptides containing repetitive RGD sequences were able to inhibit experimental and spontaneous lung metastases of B16-BL6 cells more effectively than the corresponding monomer peptides .
	manualset3
177800	1	413769	7	NULL	NULL	0	NULL	 potent inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These potent inhibitors include 70h ( GW678248 ) , which has in vitro antiviral assay IC ( 50 ) values of 0.5 nM against wild-type HIV , 1 nM against the K103N mutant associated with clinical resistance to efavirenz , and 0.7 nM against the Y181C mutant associated with clinical resistance to nevirapine .
	manualset3
177801	2	413769	7	NULL	NULL	0	NULL	70h ( GW678248 )	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	These potent inhibitors include 70h ( GW678248 ) , which has in vitro antiviral assay IC ( 50 ) values of 0.5 nM against wild-type HIV , 1 nM against the K103N mutant associated with clinical resistance to efavirenz , and 0.7 nM against the Y181C mutant associated with clinical resistance to nevirapine .
	manualset3
177802	3	413769	7	NULL	NULL	0	NULL	in vitro antiviral assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These potent inhibitors include 70h ( GW678248 ) , which has in vitro antiviral assay IC ( 50 ) values of 0.5 nM against wild-type HIV , 1 nM against the K103N mutant associated with clinical resistance to efavirenz , and 0.7 nM against the Y181C mutant associated with clinical resistance to nevirapine .
	manualset3
177803	4	413769	7	NULL	NULL	0	NULL	IC ( 50 ) values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These potent inhibitors include 70h ( GW678248 ) , which has in vitro antiviral assay IC ( 50 ) values of 0.5 nM against wild-type HIV , 1 nM against the K103N mutant associated with clinical resistance to efavirenz , and 0.7 nM against the Y181C mutant associated with clinical resistance to nevirapine .
	manualset3
177804	5	413769	7	NULL	NULL	0	NULL	0.5 nM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These potent inhibitors include 70h ( GW678248 ) , which has in vitro antiviral assay IC ( 50 ) values of 0.5 nM against wild-type HIV , 1 nM against the K103N mutant associated with clinical resistance to efavirenz , and 0.7 nM against the Y181C mutant associated with clinical resistance to nevirapine .
	manualset3
177805	6	413769	7	NULL	NULL	0	NULL	wild-type HIV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These potent inhibitors include 70h ( GW678248 ) , which has in vitro antiviral assay IC ( 50 ) values of 0.5 nM against wild-type HIV , 1 nM against the K103N mutant associated with clinical resistance to efavirenz , and 0.7 nM against the Y181C mutant associated with clinical resistance to nevirapine .
	manualset3
177806	7	413769	7	NULL	NULL	0	NULL	1 nM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These potent inhibitors include 70h ( GW678248 ) , which has in vitro antiviral assay IC ( 50 ) values of 0.5 nM against wild-type HIV , 1 nM against the K103N mutant associated with clinical resistance to efavirenz , and 0.7 nM against the Y181C mutant associated with clinical resistance to nevirapine .
	manualset3
177807	8	413769	7	NULL	NULL	0	NULL	K103N mutant	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These potent inhibitors include 70h ( GW678248 ) , which has in vitro antiviral assay IC ( 50 ) values of 0.5 nM against wild-type HIV , 1 nM against the K103N mutant associated with clinical resistance to efavirenz , and 0.7 nM against the Y181C mutant associated with clinical resistance to nevirapine .
	manualset3
177808	9	413769	7	NULL	NULL	0	NULL	clinical resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These potent inhibitors include 70h ( GW678248 ) , which has in vitro antiviral assay IC ( 50 ) values of 0.5 nM against wild-type HIV , 1 nM against the K103N mutant associated with clinical resistance to efavirenz , and 0.7 nM against the Y181C mutant associated with clinical resistance to nevirapine .
	manualset3
177809	10	413769	7	NULL	NULL	0	NULL	efavirenz	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These potent inhibitors include 70h ( GW678248 ) , which has in vitro antiviral assay IC ( 50 ) values of 0.5 nM against wild-type HIV , 1 nM against the K103N mutant associated with clinical resistance to efavirenz , and 0.7 nM against the Y181C mutant associated with clinical resistance to nevirapine .
	manualset3
177810	11	413769	7	NULL	NULL	0	NULL	0.7 nM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These potent inhibitors include 70h ( GW678248 ) , which has in vitro antiviral assay IC ( 50 ) values of 0.5 nM against wild-type HIV , 1 nM against the K103N mutant associated with clinical resistance to efavirenz , and 0.7 nM against the Y181C mutant associated with clinical resistance to nevirapine .
	manualset3
177811	12	413769	7	NULL	NULL	0	NULL	Y181C mutant	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These potent inhibitors include 70h ( GW678248 ) , which has in vitro antiviral assay IC ( 50 ) values of 0.5 nM against wild-type HIV , 1 nM against the K103N mutant associated with clinical resistance to efavirenz , and 0.7 nM against the Y181C mutant associated with clinical resistance to nevirapine .
	manualset3
177812	13	413769	7	NULL	NULL	0	NULL	clinical resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These potent inhibitors include 70h ( GW678248 ) , which has in vitro antiviral assay IC ( 50 ) values of 0.5 nM against wild-type HIV , 1 nM against the K103N mutant associated with clinical resistance to efavirenz , and 0.7 nM against the Y181C mutant associated with clinical resistance to nevirapine .
	manualset3
177813	14	413769	7	NULL	NULL	0	NULL	nevirapine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These potent inhibitors include 70h ( GW678248 ) , which has in vitro antiviral assay IC ( 50 ) values of 0.5 nM against wild-type HIV , 1 nM against the K103N mutant associated with clinical resistance to efavirenz , and 0.7 nM against the Y181C mutant associated with clinical resistance to nevirapine .
	manualset3
177814	1	413770	7	NULL	NULL	0	NULL	preliminary results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These preliminary results suggest that encapsulated islets sheets can survive and maintain islet viability and function in vivo , within the subcutaneous region .
	manualset3
177815	2	413770	7	NULL	NULL	0	NULL	encapsulated islets sheets	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These preliminary results suggest that encapsulated islets sheets can survive and maintain islet viability and function in vivo , within the subcutaneous region .
	manualset3
177816	3	413770	7	NULL	NULL	0	NULL	islet viability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These preliminary results suggest that encapsulated islets sheets can survive and maintain islet viability and function in vivo , within the subcutaneous region .
	manualset3
177817	4	413770	7	NULL	NULL	0	NULL	function 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These preliminary results suggest that encapsulated islets sheets can survive and maintain islet viability and function in vivo , within the subcutaneous region .
	manualset3
177818	5	413770	7	NULL	NULL	0	NULL	subcutaneous region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These preliminary results suggest that encapsulated islets sheets can survive and maintain islet viability and function in vivo , within the subcutaneous region .
	manualset3
177819	1	413771	7	NULL	NULL	0	NULL	probes	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These probes are examined in multiple states of the catalytic cycle of P450cam and its T252A mutant .
	manualset3
177820	2	413771	7	NULL	NULL	NULL	NULL	multiple states	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These probes are examined in multiple states of the catalytic cycle of P450cam and its T252A mutant .
	manualset3
177821	3	413771	7	NULL	NULL	NULL	NULL	catalytic cycle	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These probes are examined in multiple states of the catalytic cycle of P450cam and its T252A mutant .
	manualset3
177822	4	413771	7	NULL	NULL	0	NULL	P450cam	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These probes are examined in multiple states of the catalytic cycle of P450cam and its T252A mutant .
	manualset3
177823	5	413771	7	NULL	NULL	0	NULL	T252A mutant 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These probes are examined in multiple states of the catalytic cycle of P450cam and its T252A mutant .
	manualset3
177824	1	413772	7	NULL	NULL	0	NULL	procedures	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These procedures may be complicated by the complex anatomic relationships between cords ( pathologic contracted fascia ) and adjacent neurovascular structures .
	manualset3
177825	2	413772	7	NULL	NULL	0	NULL	complex anatomic relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These procedures may be complicated by the complex anatomic relationships between cords ( pathologic contracted fascia ) and adjacent neurovascular structures .
	manualset3
177826	3	413772	7	NULL	NULL	0	NULL	 cords	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These procedures may be complicated by the complex anatomic relationships between cords ( pathologic contracted fascia ) and adjacent neurovascular structures .
	manualset3
177827	4	413772	7	NULL	NULL	0	NULL	pathologic contracted fascia 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These procedures may be complicated by the complex anatomic relationships between cords ( pathologic contracted fascia ) and adjacent neurovascular structures .
	manualset3
177828	5	413772	7	NULL	NULL	0	NULL	neurovascular structures	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These procedures may be complicated by the complex anatomic relationships between cords ( pathologic contracted fascia ) and adjacent neurovascular structures .
	manualset3
177829	1	413773	7	NULL	NULL	0	NULL	processes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These processes are cost-intensive and also lead to the loss of the valuable phosphate resources incorporated in the sludge ash .
	manualset3
177830	2	413773	7	NULL	NULL	0	NULL	cost-intensive	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These processes are cost-intensive and also lead to the loss of the valuable phosphate resources incorporated in the sludge ash .
	manualset3
177831	3	413773	7	NULL	NULL	0	NULL	 loss	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These processes are cost-intensive and also lead to the loss of the valuable phosphate resources incorporated in the sludge ash .
	manualset3
177832	4	413773	7	NULL	NULL	0	NULL	valuable phosphate resources	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These processes are cost-intensive and also lead to the loss of the valuable phosphate resources incorporated in the sludge ash .
	manualset3
177833	5	413773	7	NULL	NULL	0	NULL	sludge ash	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These processes are cost-intensive and also lead to the loss of the valuable phosphate resources incorporated in the sludge ash .
	manualset3
177834	1	413774	7	NULL	NULL	0	NULL	products	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	These products included juices , cheeses , pasta , mushrooms , hazelnuts , sage , figs , tea , thyme , juniper , caraway seeds , and apricots .
	manualset3
177835	2	413774	7	NULL	NULL	0	NULL	juices	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	These products included juices , cheeses , pasta , mushrooms , hazelnuts , sage , figs , tea , thyme , juniper , caraway seeds , and apricots .
	manualset3
177836	3	413774	7	NULL	NULL	0	NULL	cheeses	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	These products included juices , cheeses , pasta , mushrooms , hazelnuts , sage , figs , tea , thyme , juniper , caraway seeds , and apricots .
	manualset3
177837	4	413774	7	NULL	NULL	0	NULL	pasta	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	These products included juices , cheeses , pasta , mushrooms , hazelnuts , sage , figs , tea , thyme , juniper , caraway seeds , and apricots .
	manualset3
177838	5	413774	7	NULL	NULL	0	NULL	mushrooms	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	These products included juices , cheeses , pasta , mushrooms , hazelnuts , sage , figs , tea , thyme , juniper , caraway seeds , and apricots .
	manualset3
177839	6	413774	7	NULL	NULL	0	NULL	 hazelnuts	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	These products included juices , cheeses , pasta , mushrooms , hazelnuts , sage , figs , tea , thyme , juniper , caraway seeds , and apricots .
	manualset3
177840	7	413774	7	NULL	NULL	0	NULL	sage	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	These products included juices , cheeses , pasta , mushrooms , hazelnuts , sage , figs , tea , thyme , juniper , caraway seeds , and apricots .
	manualset3
177841	8	413774	7	NULL	NULL	0	NULL	figs	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	These products included juices , cheeses , pasta , mushrooms , hazelnuts , sage , figs , tea , thyme , juniper , caraway seeds , and apricots .
	manualset3
177842	9	413774	7	NULL	NULL	0	NULL	tea	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	These products included juices , cheeses , pasta , mushrooms , hazelnuts , sage , figs , tea , thyme , juniper , caraway seeds , and apricots .
	manualset3
177843	10	413774	7	NULL	NULL	0	NULL	thyme	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	These products included juices , cheeses , pasta , mushrooms , hazelnuts , sage , figs , tea , thyme , juniper , caraway seeds , and apricots .
	manualset3
177844	11	413774	7	NULL	NULL	0	NULL	 juniper	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	These products included juices , cheeses , pasta , mushrooms , hazelnuts , sage , figs , tea , thyme , juniper , caraway seeds , and apricots .
	manualset3
177845	12	413774	7	NULL	NULL	0	NULL	 caraway seeds	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	These products included juices , cheeses , pasta , mushrooms , hazelnuts , sage , figs , tea , thyme , juniper , caraway seeds , and apricots .
	manualset3
177846	13	413774	7	NULL	NULL	0	NULL	apricots	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	These products included juices , cheeses , pasta , mushrooms , hazelnuts , sage , figs , tea , thyme , juniper , caraway seeds , and apricots .
	manualset3
177847	1	413775	7	NULL	NULL	0	NULL	properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These properties provide characteristics for the identification and classification of biological systems ranging in size and composition from proteins and nucleic acids to cells .
	manualset3
177848	2	413775	7	NULL	NULL	0	NULL	 identification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These properties provide characteristics for the identification and classification of biological systems ranging in size and composition from proteins and nucleic acids to cells .
	manualset3
177849	3	413775	7	NULL	NULL	0	NULL	classification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These properties provide characteristics for the identification and classification of biological systems ranging in size and composition from proteins and nucleic acids to cells .
	manualset3
177850	4	413775	7	NULL	NULL	0	NULL	biological systems	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These properties provide characteristics for the identification and classification of biological systems ranging in size and composition from proteins and nucleic acids to cells .
	manualset3
177851	5	413775	7	NULL	NULL	0	NULL	size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These properties provide characteristics for the identification and classification of biological systems ranging in size and composition from proteins and nucleic acids to cells .
	manualset3
177852	6	413775	7	NULL	NULL	0	NULL	composition	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These properties provide characteristics for the identification and classification of biological systems ranging in size and composition from proteins and nucleic acids to cells .
	manualset3
177853	7	413775	7	NULL	NULL	0	NULL	proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These properties provide characteristics for the identification and classification of biological systems ranging in size and composition from proteins and nucleic acids to cells .
	manualset3
177854	8	413775	7	NULL	NULL	0	NULL	nucleic acids	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These properties provide characteristics for the identification and classification of biological systems ranging in size and composition from proteins and nucleic acids to cells .
	manualset3
177855	9	413775	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These properties provide characteristics for the identification and classification of biological systems ranging in size and composition from proteins and nucleic acids to cells .
	manualset3
177856	10	413775	7	NULL	NULL	0	NULL	characteristics	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These properties provide characteristics for the identification and classification of biological systems ranging in size and composition from proteins and nucleic acids to cells .
	manualset3
177857	1	413776	7	NULL	NULL	0	NULL	protein-DNA interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These protein-DNA interactions persist during all phases of the cell cycle and dissociate with 0.16 to 0.2 M sodium chloride .
	manualset3
177858	2	413776	7	NULL	NULL	0	NULL	phases	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These protein-DNA interactions persist during all phases of the cell cycle and dissociate with 0.16 to 0.2 M sodium chloride .
	manualset3
177859	3	413776	7	NULL	NULL	0	NULL	cell cycle	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These protein-DNA interactions persist during all phases of the cell cycle and dissociate with 0.16 to 0.2 M sodium chloride .
	manualset3
177860	4	413776	7	NULL	NULL	0	NULL	0.16 M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These protein-DNA interactions persist during all phases of the cell cycle and dissociate with 0.16 to 0.2 M sodium chloride .
	manualset3
177861	5	413776	7	NULL	NULL	0	NULL	0.2 M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These protein-DNA interactions persist during all phases of the cell cycle and dissociate with 0.16 to 0.2 M sodium chloride .
	manualset3
177862	6	413776	7	NULL	NULL	0	NULL	sodium chloride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These protein-DNA interactions persist during all phases of the cell cycle and dissociate with 0.16 to 0.2 M sodium chloride .
	manualset3
177863	1	413777	7	NULL	NULL	0	NULL	proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These proteins , whose secondary structures are predominantly alpha-helical segments , and many peptides form pores in membranes without a crystallizable protein assembly , contrary to the family of beta-pore-forming proteins , which form crystallizable beta-barrel pores .
	manualset3
177864	2	413777	7	NULL	NULL	0	NULL	secondary structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These proteins , whose secondary structures are predominantly alpha-helical segments , and many peptides form pores in membranes without a crystallizable protein assembly , contrary to the family of beta-pore-forming proteins , which form crystallizable beta-barrel pores .
	manualset3
177865	3	413777	7	NULL	NULL	0	NULL	alpha-helical segments 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These proteins , whose secondary structures are predominantly alpha-helical segments , and many peptides form pores in membranes without a crystallizable protein assembly , contrary to the family of beta-pore-forming proteins , which form crystallizable beta-barrel pores .
	manualset3
177866	4	413777	7	NULL	NULL	0	NULL	 peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	These proteins , whose secondary structures are predominantly alpha-helical segments , and many peptides form pores in membranes without a crystallizable protein assembly , contrary to the family of beta-pore-forming proteins , which form crystallizable beta-barrel pores .
	manualset3
177867	5	413777	7	NULL	NULL	0	NULL	pores	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These proteins , whose secondary structures are predominantly alpha-helical segments , and many peptides form pores in membranes without a crystallizable protein assembly , contrary to the family of beta-pore-forming proteins , which form crystallizable beta-barrel pores .
	manualset3
177868	6	413777	7	NULL	NULL	0	NULL	membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These proteins , whose secondary structures are predominantly alpha-helical segments , and many peptides form pores in membranes without a crystallizable protein assembly , contrary to the family of beta-pore-forming proteins , which form crystallizable beta-barrel pores .
	manualset3
177869	7	413777	7	NULL	NULL	0	NULL	crystallizable protein assembly	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These proteins , whose secondary structures are predominantly alpha-helical segments , and many peptides form pores in membranes without a crystallizable protein assembly , contrary to the family of beta-pore-forming proteins , which form crystallizable beta-barrel pores .
	manualset3
177870	8	413777	7	NULL	NULL	0	NULL	family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These proteins , whose secondary structures are predominantly alpha-helical segments , and many peptides form pores in membranes without a crystallizable protein assembly , contrary to the family of beta-pore-forming proteins , which form crystallizable beta-barrel pores .
	manualset3
177871	9	413777	7	NULL	NULL	0	NULL	 beta-pore-forming proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These proteins , whose secondary structures are predominantly alpha-helical segments , and many peptides form pores in membranes without a crystallizable protein assembly , contrary to the family of beta-pore-forming proteins , which form crystallizable beta-barrel pores .
	manualset3
177872	10	413777	7	NULL	NULL	0	NULL	crystallizable beta-barrel pores	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These proteins , whose secondary structures are predominantly alpha-helical segments , and many peptides form pores in membranes without a crystallizable protein assembly , contrary to the family of beta-pore-forming proteins , which form crystallizable beta-barrel pores .
	manualset3
177873	1	413778	7	NULL	NULL	0	NULL	deletional analysis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional deletional analysis showed that the SH3 domain was not required for inhibition of lamellipod extension , as a construct containing only the proline-rich and breakpoint cluster region ( BCR ) homology domains was sufficient for inhibition .
	manualset3
177874	2	413778	7	NULL	NULL	0	NULL	SH3 domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional deletional analysis showed that the SH3 domain was not required for inhibition of lamellipod extension , as a construct containing only the proline-rich and breakpoint cluster region ( BCR ) homology domains was sufficient for inhibition .
	manualset3
177875	3	413778	7	NULL	NULL	0	NULL	 inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional deletional analysis showed that the SH3 domain was not required for inhibition of lamellipod extension , as a construct containing only the proline-rich and breakpoint cluster region ( BCR ) homology domains was sufficient for inhibition .
	manualset3
177876	4	413778	7	NULL	NULL	0	NULL	lamellipod extension	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional deletional analysis showed that the SH3 domain was not required for inhibition of lamellipod extension , as a construct containing only the proline-rich and breakpoint cluster region ( BCR ) homology domains was sufficient for inhibition .
	manualset3
177877	5	413778	7	NULL	NULL	0	NULL	construct 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional deletional analysis showed that the SH3 domain was not required for inhibition of lamellipod extension , as a construct containing only the proline-rich and breakpoint cluster region ( BCR ) homology domains was sufficient for inhibition .
	manualset3
177878	6	413778	7	NULL	NULL	0	NULL	proline-rich homology domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional deletional analysis showed that the SH3 domain was not required for inhibition of lamellipod extension , as a construct containing only the proline-rich and breakpoint cluster region ( BCR ) homology domains was sufficient for inhibition .
	manualset3
177879	7	413778	7	NULL	NULL	0	NULL	breakpoint cluster region ( BCR ) homology domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional deletional analysis showed that the SH3 domain was not required for inhibition of lamellipod extension , as a construct containing only the proline-rich and breakpoint cluster region ( BCR ) homology domains was sufficient for inhibition .
	manualset3
177880	8	413778	7	NULL	NULL	0	NULL	inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional deletional analysis showed that the SH3 domain was not required for inhibition of lamellipod extension , as a construct containing only the proline-rich and breakpoint cluster region ( BCR ) homology domains was sufficient for inhibition .
	manualset3
177881	1	413779	7	NULL	NULL	0	NULL	 proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These proteins also have been shown to have early meiotic roles essential for the formation of a programmed DNA double-strand break known in Saccharomyces cerevisiae to initiate meiotic recombination .
	manualset3
177882	2	413779	7	NULL	NULL	0	NULL	early meiotic roles	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These proteins also have been shown to have early meiotic roles essential for the formation of a programmed DNA double-strand break known in Saccharomyces cerevisiae to initiate meiotic recombination .
	manualset3
177883	3	413779	7	NULL	NULL	0	NULL	 formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These proteins also have been shown to have early meiotic roles essential for the formation of a programmed DNA double-strand break known in Saccharomyces cerevisiae to initiate meiotic recombination .
	manualset3
177884	4	413779	7	NULL	NULL	0	NULL	programmed DNA double-strand break	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These proteins also have been shown to have early meiotic roles essential for the formation of a programmed DNA double-strand break known in Saccharomyces cerevisiae to initiate meiotic recombination .
	manualset3
177885	5	413779	7	NULL	NULL	0	NULL	Saccharomyces cerevisiae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These proteins also have been shown to have early meiotic roles essential for the formation of a programmed DNA double-strand break known in Saccharomyces cerevisiae to initiate meiotic recombination .
	manualset3
177886	6	413779	7	NULL	NULL	0	NULL	meiotic recombination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These proteins also have been shown to have early meiotic roles essential for the formation of a programmed DNA double-strand break known in Saccharomyces cerevisiae to initiate meiotic recombination .
	manualset3
177887	1	413780	7	NULL	NULL	0	NULL	proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These proteins were designated as such because when overexpressed , host cells exhibited higher rates of accretion of radioactive or fluorescent fatty acids .
	manualset3
177888	2	413780	7	NULL	NULL	0	NULL	 host cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These proteins were designated as such because when overexpressed , host cells exhibited higher rates of accretion of radioactive or fluorescent fatty acids .
	manualset3
177889	3	413780	7	NULL	NULL	0	NULL	higher rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These proteins were designated as such because when overexpressed , host cells exhibited higher rates of accretion of radioactive or fluorescent fatty acids .
	manualset3
177890	4	413780	7	NULL	NULL	0	NULL	accretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These proteins were designated as such because when overexpressed , host cells exhibited higher rates of accretion of radioactive or fluorescent fatty acids .
	manualset3
177891	5	413780	7	NULL	NULL	0	NULL	radioactive fatty acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These proteins were designated as such because when overexpressed , host cells exhibited higher rates of accretion of radioactive or fluorescent fatty acids .
	manualset3
177892	6	413780	7	NULL	NULL	0	NULL	fluorescent fatty acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These proteins were designated as such because when overexpressed , host cells exhibited higher rates of accretion of radioactive or fluorescent fatty acids .
	manualset3
177893	1	413781	7	NULL	NULL	0	NULL	 rates 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These rates can be estimated from features of pretreatment MR images and can be applied in a mathematical model to predict tumor growth , impact of extent of tumor resection and patient survival .
	manualset3
177894	2	413781	7	NULL	NULL	0	NULL	features	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These rates can be estimated from features of pretreatment MR images and can be applied in a mathematical model to predict tumor growth , impact of extent of tumor resection and patient survival .
	manualset3
177895	3	413781	7	NULL	NULL	0	NULL	pretreatment MR images	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These rates can be estimated from features of pretreatment MR images and can be applied in a mathematical model to predict tumor growth , impact of extent of tumor resection and patient survival .
	manualset3
177896	4	413781	7	NULL	NULL	0	NULL	mathematical model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These rates can be estimated from features of pretreatment MR images and can be applied in a mathematical model to predict tumor growth , impact of extent of tumor resection and patient survival .
	manualset3
177897	5	413781	7	NULL	NULL	0	NULL	 tumor growth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These rates can be estimated from features of pretreatment MR images and can be applied in a mathematical model to predict tumor growth , impact of extent of tumor resection and patient survival .
	manualset3
177898	6	413781	7	NULL	NULL	0	NULL	impact	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These rates can be estimated from features of pretreatment MR images and can be applied in a mathematical model to predict tumor growth , impact of extent of tumor resection and patient survival .
	manualset3
177899	7	413781	7	NULL	NULL	0	NULL	extent	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These rates can be estimated from features of pretreatment MR images and can be applied in a mathematical model to predict tumor growth , impact of extent of tumor resection and patient survival .
	manualset3
177900	8	413781	7	NULL	NULL	0	NULL	tumor resection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These rates can be estimated from features of pretreatment MR images and can be applied in a mathematical model to predict tumor growth , impact of extent of tumor resection and patient survival .
	manualset3
177901	9	413781	7	NULL	NULL	0	NULL	patient survival 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These rates can be estimated from features of pretreatment MR images and can be applied in a mathematical model to predict tumor growth , impact of extent of tumor resection and patient survival .
	manualset3
177902	1	413782	7	NULL	NULL	0	NULL	 rates of release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These rates of release indicate that the HCG produced by the early placenta was rapidly passed into the circulation rather than stored .
	manualset3
177903	2	413782	7	NULL	NULL	0	NULL	HCG	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These rates of release indicate that the HCG produced by the early placenta was rapidly passed into the circulation rather than stored .
	manualset3
177904	3	413782	7	NULL	NULL	0	NULL	early placenta	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These rates of release indicate that the HCG produced by the early placenta was rapidly passed into the circulation rather than stored .
	manualset3
177905	4	413782	7	NULL	NULL	0	NULL	circulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These rates of release indicate that the HCG produced by the early placenta was rapidly passed into the circulation rather than stored .
	manualset3
177906	1	413783	7	NULL	NULL	0	NULL	 closer to the field ' methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These recently developed ` closer to the field ' methods allow rapid detection of influenza viruses and the identification of pathogenicity variants .
	manualset3
177907	2	413783	7	NULL	NULL	0	NULL	detection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These recently developed ` closer to the field ' methods allow rapid detection of influenza viruses and the identification of pathogenicity variants .
	manualset3
177908	3	413783	7	NULL	NULL	0	NULL	influenza viruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These recently developed ` closer to the field ' methods allow rapid detection of influenza viruses and the identification of pathogenicity variants .
	manualset3
177909	4	413783	7	NULL	NULL	0	NULL	identification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These recently developed ` closer to the field ' methods allow rapid detection of influenza viruses and the identification of pathogenicity variants .
	manualset3
177910	5	413783	7	NULL	NULL	0	NULL	pathogenicity variants	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These recently developed ` closer to the field ' methods allow rapid detection of influenza viruses and the identification of pathogenicity variants .
	manualset3
177911	1	413784	7	NULL	NULL	0	NULL	receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These receptors , which remain tyrosine-phosphorylated despite the addition of hapten , are progressively targeted to a Triton X-100-insoluble fraction , suggesting their progressive association with the membrane skeleton .
	manualset3
177912	2	413784	7	NULL	NULL	0	NULL	addition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These receptors , which remain tyrosine-phosphorylated despite the addition of hapten , are progressively targeted to a Triton X-100-insoluble fraction , suggesting their progressive association with the membrane skeleton .
	manualset3
177913	3	413784	7	NULL	NULL	0	NULL	hapten	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These receptors , which remain tyrosine-phosphorylated despite the addition of hapten , are progressively targeted to a Triton X-100-insoluble fraction , suggesting their progressive association with the membrane skeleton .
	manualset3
177914	4	413784	7	NULL	NULL	0	NULL	Triton X-100-insoluble fraction	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These receptors , which remain tyrosine-phosphorylated despite the addition of hapten , are progressively targeted to a Triton X-100-insoluble fraction , suggesting their progressive association with the membrane skeleton .
	manualset3
177915	5	413784	7	NULL	NULL	0	NULL	progressive association	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These receptors , which remain tyrosine-phosphorylated despite the addition of hapten , are progressively targeted to a Triton X-100-insoluble fraction , suggesting their progressive association with the membrane skeleton .
	manualset3
177916	6	413784	7	NULL	NULL	0	NULL	 membrane skeleton	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These receptors , which remain tyrosine-phosphorylated despite the addition of hapten , are progressively targeted to a Triton X-100-insoluble fraction , suggesting their progressive association with the membrane skeleton .
	manualset3
177917	1	413785	7	NULL	NULL	0	NULL	receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These receptors include specific receptors for IgG or IgA and complement receptors .
	manualset3
177918	2	413785	7	NULL	NULL	0	NULL	receptors for IgG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These receptors include specific receptors for IgG or IgA and complement receptors .
	manualset3
177919	3	413785	7	NULL	NULL	NULL	NULL	receptors for IgA	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These receptors include specific receptors for IgG or IgA and complement receptors .
	manualset3
177920	4	413785	7	NULL	NULL	NULL	NULL	complement receptors	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These receptors include specific receptors for IgG or IgA and complement receptors .
	manualset3
177921	1	413786	7	NULL	NULL	0	NULL	 regulatory effects 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These regulatory effects of highly elevated tocopherols on tissue inflammation and lung lavage fluid were reversible in a second phase of Ag challenge without tocopherols .
	manualset3
177922	2	413786	7	NULL	NULL	0	NULL	 highly elevated tocopherols	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These regulatory effects of highly elevated tocopherols on tissue inflammation and lung lavage fluid were reversible in a second phase of Ag challenge without tocopherols .
	manualset3
177923	3	413786	7	NULL	NULL	0	NULL	tissue inflammation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These regulatory effects of highly elevated tocopherols on tissue inflammation and lung lavage fluid were reversible in a second phase of Ag challenge without tocopherols .
	manualset3
177924	4	413786	7	NULL	NULL	0	NULL	 lung lavage fluid 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These regulatory effects of highly elevated tocopherols on tissue inflammation and lung lavage fluid were reversible in a second phase of Ag challenge without tocopherols .
	manualset3
177925	5	413786	7	NULL	NULL	0	NULL	second phase	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	These regulatory effects of highly elevated tocopherols on tissue inflammation and lung lavage fluid were reversible in a second phase of Ag challenge without tocopherols .
	manualset3
177926	6	413786	7	NULL	NULL	0	NULL	Ag challenge	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These regulatory effects of highly elevated tocopherols on tissue inflammation and lung lavage fluid were reversible in a second phase of Ag challenge without tocopherols .
	manualset3
177927	7	413786	7	NULL	NULL	0	NULL	tocopherols	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These regulatory effects of highly elevated tocopherols on tissue inflammation and lung lavage fluid were reversible in a second phase of Ag challenge without tocopherols .
	manualset3
177928	1	413787	7	NULL	NULL	0	NULL	 relations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These relations were compared with results of variable-temperature 13C solid-state NMR observation of beeswax .
	manualset3
177929	2	413787	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These relations were compared with results of variable-temperature 13C solid-state NMR observation of beeswax .
	manualset3
177930	3	413787	7	NULL	NULL	0	NULL	variable-temperature 13C solid-state NMR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These relations were compared with results of variable-temperature 13C solid-state NMR observation of beeswax .
	manualset3
177931	4	413787	7	NULL	NULL	0	NULL	observation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These relations were compared with results of variable-temperature 13C solid-state NMR observation of beeswax .
	manualset3
177932	5	413787	7	NULL	NULL	NULL	NULL	beeswax	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These relations were compared with results of variable-temperature 13C solid-state NMR observation of beeswax .
	manualset3
177933	1	413788	7	NULL	NULL	0	NULL	 relations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These relations were similar in all age groups and are suggested to be properties intrinsic to the IFS MNs .
	manualset3
177934	2	413788	7	NULL	NULL	0	NULL	age groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These relations were similar in all age groups and are suggested to be properties intrinsic to the IFS MNs .
	manualset3
177935	3	413788	7	NULL	NULL	0	NULL	IFS MNs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These relations were similar in all age groups and are suggested to be properties intrinsic to the IFS MNs .
	manualset3
177940	4	413788	7	NULL	NULL	0	NULL	properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These relations were similar in all age groups and are suggested to be properties intrinsic to the IFS MNs .
	manualset3
177936	1	413789	7	NULL	NULL	0	NULL	relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These relationships depend on the complexities of both the classifier and the data .
	manualset3
177937	2	413789	7	NULL	NULL	0	NULL	complexities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These relationships depend on the complexities of both the classifier and the data .
	manualset3
177938	3	413789	7	NULL	NULL	0	NULL	classifier	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These relationships depend on the complexities of both the classifier and the data .
	manualset3
177939	4	413789	7	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These relationships depend on the complexities of both the classifier and the data .
	manualset3
177941	1	413790	7	NULL	NULL	0	NULL	researchers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These researchers emphasized the incentives for human capital formation in the source country .
	manualset3
177942	2	413790	7	NULL	NULL	0	NULL	 incentives	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These researchers emphasized the incentives for human capital formation in the source country .
	manualset3
177943	3	413790	7	NULL	NULL	0	NULL	human capital formation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These researchers emphasized the incentives for human capital formation in the source country .
	manualset3
177945	4	413790	7	NULL	NULL	0	NULL	source country	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	These researchers emphasized the incentives for human capital formation in the source country .
	manualset3
177946	1	413791	7	NULL	NULL	0	NULL	responses 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These responses are competitively antagonized by atropine and phentolamine or yohimbine respectively .
	manualset3
177947	2	413791	7	NULL	NULL	0	NULL	atropine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These responses are competitively antagonized by atropine and phentolamine or yohimbine respectively .
	manualset3
177948	3	413791	7	NULL	NULL	0	NULL	phentolamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These responses are competitively antagonized by atropine and phentolamine or yohimbine respectively .
	manualset3
177949	4	413791	7	NULL	NULL	0	NULL	yohimbine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These responses are competitively antagonized by atropine and phentolamine or yohimbine respectively .
	manualset3
177950	1	413792	7	NULL	NULL	0	NULL	responses 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These responses were potentiated when preparations were previously incubated with thiorphan ( 10 microM ) , an inhibitor of tachykinin breakdown , but were significantly depressed when sensory nerves were previously desensitized in vitro by capsaicin ( 10 microM for 15 min ) challenge .
	manualset3
177951	2	413792	7	NULL	NULL	0	NULL	preparations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These responses were potentiated when preparations were previously incubated with thiorphan ( 10 microM ) , an inhibitor of tachykinin breakdown , but were significantly depressed when sensory nerves were previously desensitized in vitro by capsaicin ( 10 microM for 15 min ) challenge .
	manualset3
177952	3	413792	7	NULL	NULL	NULL	NULL	 thiorphan 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These responses were potentiated when preparations were previously incubated with thiorphan ( 10 microM ) , an inhibitor of tachykinin breakdown , but were significantly depressed when sensory nerves were previously desensitized in vitro by capsaicin ( 10 microM for 15 min ) challenge .
	manualset3
177953	4	413792	7	NULL	NULL	0	NULL	10 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These responses were potentiated when preparations were previously incubated with thiorphan ( 10 microM ) , an inhibitor of tachykinin breakdown , but were significantly depressed when sensory nerves were previously desensitized in vitro by capsaicin ( 10 microM for 15 min ) challenge .
	manualset3
177954	5	413792	7	NULL	NULL	0	NULL	inhibitor 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These responses were potentiated when preparations were previously incubated with thiorphan ( 10 microM ) , an inhibitor of tachykinin breakdown , but were significantly depressed when sensory nerves were previously desensitized in vitro by capsaicin ( 10 microM for 15 min ) challenge .
	manualset3
177955	6	413792	7	NULL	NULL	0	NULL	tachykinin breakdown 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These responses were potentiated when preparations were previously incubated with thiorphan ( 10 microM ) , an inhibitor of tachykinin breakdown , but were significantly depressed when sensory nerves were previously desensitized in vitro by capsaicin ( 10 microM for 15 min ) challenge .
	manualset3
177956	7	413792	7	NULL	NULL	0	NULL	sensory nerves	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These responses were potentiated when preparations were previously incubated with thiorphan ( 10 microM ) , an inhibitor of tachykinin breakdown , but were significantly depressed when sensory nerves were previously desensitized in vitro by capsaicin ( 10 microM for 15 min ) challenge .
	manualset3
177957	8	413792	7	NULL	NULL	NULL	NULL	capsaicin challenge	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These responses were potentiated when preparations were previously incubated with thiorphan ( 10 microM ) , an inhibitor of tachykinin breakdown , but were significantly depressed when sensory nerves were previously desensitized in vitro by capsaicin ( 10 microM for 15 min ) challenge .
	manualset3
177958	9	413792	7	NULL	NULL	0	NULL	10 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These responses were potentiated when preparations were previously incubated with thiorphan ( 10 microM ) , an inhibitor of tachykinin breakdown , but were significantly depressed when sensory nerves were previously desensitized in vitro by capsaicin ( 10 microM for 15 min ) challenge .
	manualset3
177959	10	413792	7	NULL	NULL	0	NULL	15 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	These responses were potentiated when preparations were previously incubated with thiorphan ( 10 microM ) , an inhibitor of tachykinin breakdown , but were significantly depressed when sensory nerves were previously desensitized in vitro by capsaicin ( 10 microM for 15 min ) challenge .
	manualset3
177961	1	413793	7	NULL	NULL	0	NULL	constant area	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These result in 3 ) a constant area of irradiation ( one square centimeter ) , and 4 ) an irradiated area that is clearly distinguished by the ring .
	manualset3
177962	2	413793	7	NULL	NULL	0	NULL	irradiation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These result in 3 ) a constant area of irradiation ( one square centimeter ) , and 4 ) an irradiated area that is clearly distinguished by the ring .
	manualset3
177963	3	413793	7	NULL	NULL	0	NULL	one square centimeter 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These result in 3 ) a constant area of irradiation ( one square centimeter ) , and 4 ) an irradiated area that is clearly distinguished by the ring .
	manualset3
177964	4	413793	7	NULL	NULL	0	NULL	irradiated area	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These result in 3 ) a constant area of irradiation ( one square centimeter ) , and 4 ) an irradiated area that is clearly distinguished by the ring .
	manualset3
177965	5	413793	7	NULL	NULL	0	NULL	 ring	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These result in 3 ) a constant area of irradiation ( one square centimeter ) , and 4 ) an irradiated area that is clearly distinguished by the ring .
	manualset3
177966	1	413794	7	NULL	NULL	0	NULL	mutants	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional mutants were isolated by site-directed mutagenesis followed by genetic selection ; the mutant enzymes have single amino acid changes ( Lys-317 -- ) Arg and Gln-318 -- ) Lys ) .
	manualset3
177967	2	413794	7	NULL	NULL	NULL	NULL	site-directed mutagenesis	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Additional mutants were isolated by site-directed mutagenesis followed by genetic selection ; the mutant enzymes have single amino acid changes ( Lys-317 -- ) Arg and Gln-318 -- ) Lys ) .
	manualset3
177968	3	413794	7	NULL	NULL	0	NULL	genetic selection	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional mutants were isolated by site-directed mutagenesis followed by genetic selection ; the mutant enzymes have single amino acid changes ( Lys-317 -- ) Arg and Gln-318 -- ) Lys ) .
	manualset3
177969	4	413794	7	NULL	NULL	0	NULL	mutant enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional mutants were isolated by site-directed mutagenesis followed by genetic selection ; the mutant enzymes have single amino acid changes ( Lys-317 -- ) Arg and Gln-318 -- ) Lys ) .
	manualset3
177970	5	413794	7	NULL	NULL	0	NULL	single amino acid changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional mutants were isolated by site-directed mutagenesis followed by genetic selection ; the mutant enzymes have single amino acid changes ( Lys-317 -- ) Arg and Gln-318 -- ) Lys ) .
	manualset3
177971	6	413794	7	NULL	NULL	NULL	NULL	( Lys-317 -- ) Arg and Gln-318 -- ) Lys )	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Additional mutants were isolated by site-directed mutagenesis followed by genetic selection ; the mutant enzymes have single amino acid changes ( Lys-317 -- ) Arg and Gln-318 -- ) Lys ) .
	manualset3
177972	1	413795	7	NULL	NULL	NULL	NULL	combination 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results , in combination with previous work , suggest that muscle rigidity , a clinically relevant side-effect of parenteral narcotic administration , may be partly mediated via serotonergic pathways .
	manualset3
177973	2	413795	7	NULL	NULL	0	NULL	previous work	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , in combination with previous work , suggest that muscle rigidity , a clinically relevant side-effect of parenteral narcotic administration , may be partly mediated via serotonergic pathways .
	manualset3
177974	3	413795	7	NULL	NULL	0	NULL	muscle rigidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , in combination with previous work , suggest that muscle rigidity , a clinically relevant side-effect of parenteral narcotic administration , may be partly mediated via serotonergic pathways .
	manualset3
177975	4	413795	7	NULL	NULL	0	NULL	side-effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , in combination with previous work , suggest that muscle rigidity , a clinically relevant side-effect of parenteral narcotic administration , may be partly mediated via serotonergic pathways .
	manualset3
177976	5	413795	7	NULL	NULL	0	NULL	parenteral narcotic administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , in combination with previous work , suggest that muscle rigidity , a clinically relevant side-effect of parenteral narcotic administration , may be partly mediated via serotonergic pathways .
	manualset3
177977	6	413795	7	NULL	NULL	0	NULL	serotonergic pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , in combination with previous work , suggest that muscle rigidity , a clinically relevant side-effect of parenteral narcotic administration , may be partly mediated via serotonergic pathways .
	manualset3
177978	1	413796	7	NULL	NULL	0	NULL	combination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , in combination with the ability of heparin and chondroitin sulfate to compete for binding to DNs , demonstrate that these two glycosaminoglycans interact with similar or overlapping sites in FN .
	manualset3
177979	2	413796	7	NULL	NULL	0	NULL	ability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , in combination with the ability of heparin and chondroitin sulfate to compete for binding to DNs , demonstrate that these two glycosaminoglycans interact with similar or overlapping sites in FN .
	manualset3
177980	3	413796	7	NULL	NULL	0	NULL	heparin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , in combination with the ability of heparin and chondroitin sulfate to compete for binding to DNs , demonstrate that these two glycosaminoglycans interact with similar or overlapping sites in FN .
	manualset3
177981	4	413796	7	NULL	NULL	0	NULL	chondroitin sulfate	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , in combination with the ability of heparin and chondroitin sulfate to compete for binding to DNs , demonstrate that these two glycosaminoglycans interact with similar or overlapping sites in FN .
	manualset3
177982	5	413796	7	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , in combination with the ability of heparin and chondroitin sulfate to compete for binding to DNs , demonstrate that these two glycosaminoglycans interact with similar or overlapping sites in FN .
	manualset3
177983	6	413796	7	NULL	NULL	0	NULL	DNs	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , in combination with the ability of heparin and chondroitin sulfate to compete for binding to DNs , demonstrate that these two glycosaminoglycans interact with similar or overlapping sites in FN .
	manualset3
177984	7	413796	7	NULL	NULL	0	NULL	glycosaminoglycans	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , in combination with the ability of heparin and chondroitin sulfate to compete for binding to DNs , demonstrate that these two glycosaminoglycans interact with similar or overlapping sites in FN .
	manualset3
177985	8	413796	7	NULL	NULL	0	NULL	overlapping sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , in combination with the ability of heparin and chondroitin sulfate to compete for binding to DNs , demonstrate that these two glycosaminoglycans interact with similar or overlapping sites in FN .
	manualset3
177986	9	413796	7	NULL	NULL	0	NULL	FN	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , in combination with the ability of heparin and chondroitin sulfate to compete for binding to DNs , demonstrate that these two glycosaminoglycans interact with similar or overlapping sites in FN .
	manualset3
177987	1	413797	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , therefore , unambiguously confirmed the capacity of the decidualized cells of maternal origin to express P450scc mRNA and , thus , ruled out any direct role of the blastocyst involvement in P450scc induction .
	manualset3
177988	2	413797	7	NULL	NULL	0	NULL	capacity 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , therefore , unambiguously confirmed the capacity of the decidualized cells of maternal origin to express P450scc mRNA and , thus , ruled out any direct role of the blastocyst involvement in P450scc induction .
	manualset3
177989	3	413797	7	NULL	NULL	0	NULL	decidualized cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , therefore , unambiguously confirmed the capacity of the decidualized cells of maternal origin to express P450scc mRNA and , thus , ruled out any direct role of the blastocyst involvement in P450scc induction .
	manualset3
177990	4	413797	7	NULL	NULL	0	NULL	maternal origin	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , therefore , unambiguously confirmed the capacity of the decidualized cells of maternal origin to express P450scc mRNA and , thus , ruled out any direct role of the blastocyst involvement in P450scc induction .
	manualset3
177991	5	413797	7	NULL	NULL	0	NULL	P450scc mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , therefore , unambiguously confirmed the capacity of the decidualized cells of maternal origin to express P450scc mRNA and , thus , ruled out any direct role of the blastocyst involvement in P450scc induction .
	manualset3
177992	6	413797	7	NULL	NULL	0	NULL	 role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , therefore , unambiguously confirmed the capacity of the decidualized cells of maternal origin to express P450scc mRNA and , thus , ruled out any direct role of the blastocyst involvement in P450scc induction .
	manualset3
177993	7	413797	7	NULL	NULL	0	NULL	blastocyst involvement	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , therefore , unambiguously confirmed the capacity of the decidualized cells of maternal origin to express P450scc mRNA and , thus , ruled out any direct role of the blastocyst involvement in P450scc induction .
	manualset3
177994	8	413797	7	NULL	NULL	0	NULL	P450scc	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , therefore , unambiguously confirmed the capacity of the decidualized cells of maternal origin to express P450scc mRNA and , thus , ruled out any direct role of the blastocyst involvement in P450scc induction .
	manualset3
177995	9	413797	7	NULL	NULL	0	NULL	induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , therefore , unambiguously confirmed the capacity of the decidualized cells of maternal origin to express P450scc mRNA and , thus , ruled out any direct role of the blastocyst involvement in P450scc induction .
	manualset3
177996	1	413798	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , together with morphological observations indicate that , at the de-differentiation stage , CAPE stimulated wound re-epithelization , increased keratinocyte proliferation and increased thickness of the wound epidermis .
	manualset3
177997	2	413798	7	NULL	NULL	0	NULL	morphological observations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , together with morphological observations indicate that , at the de-differentiation stage , CAPE stimulated wound re-epithelization , increased keratinocyte proliferation and increased thickness of the wound epidermis .
	manualset3
177998	3	413798	7	NULL	NULL	0	NULL	de-differentiation stage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , together with morphological observations indicate that , at the de-differentiation stage , CAPE stimulated wound re-epithelization , increased keratinocyte proliferation and increased thickness of the wound epidermis .
	manualset3
177999	4	413798	7	NULL	NULL	0	NULL	CAPE	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , together with morphological observations indicate that , at the de-differentiation stage , CAPE stimulated wound re-epithelization , increased keratinocyte proliferation and increased thickness of the wound epidermis .
	manualset3
178000	5	413798	7	NULL	NULL	0	NULL	wound re-epithelization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , together with morphological observations indicate that , at the de-differentiation stage , CAPE stimulated wound re-epithelization , increased keratinocyte proliferation and increased thickness of the wound epidermis .
	manualset3
178001	6	413798	7	NULL	NULL	0	NULL	keratinocyte proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , together with morphological observations indicate that , at the de-differentiation stage , CAPE stimulated wound re-epithelization , increased keratinocyte proliferation and increased thickness of the wound epidermis .
	manualset3
178002	7	413798	7	NULL	NULL	0	NULL	thickness 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , together with morphological observations indicate that , at the de-differentiation stage , CAPE stimulated wound re-epithelization , increased keratinocyte proliferation and increased thickness of the wound epidermis .
	manualset3
178003	8	413798	7	NULL	NULL	0	NULL	wound epidermis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results , together with morphological observations indicate that , at the de-differentiation stage , CAPE stimulated wound re-epithelization , increased keratinocyte proliferation and increased thickness of the wound epidermis .
	manualset3
178004	1	413799	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results add evidence that among the selected markers supposed to be relevant for melanoma progression the presence of dipeptidyl peptidase IV can be used to support diagnosis of deep penetrating nevi in doubtful cases .
	manualset3
178005	2	413799	7	NULL	NULL	0	NULL	evidence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results add evidence that among the selected markers supposed to be relevant for melanoma progression the presence of dipeptidyl peptidase IV can be used to support diagnosis of deep penetrating nevi in doubtful cases .
	manualset3
178006	3	413799	7	NULL	NULL	0	NULL	selected markers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results add evidence that among the selected markers supposed to be relevant for melanoma progression the presence of dipeptidyl peptidase IV can be used to support diagnosis of deep penetrating nevi in doubtful cases .
	manualset3
178007	4	413799	7	NULL	NULL	0	NULL	melanoma progression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results add evidence that among the selected markers supposed to be relevant for melanoma progression the presence of dipeptidyl peptidase IV can be used to support diagnosis of deep penetrating nevi in doubtful cases .
	manualset3
178008	5	413799	7	NULL	NULL	0	NULL	presence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results add evidence that among the selected markers supposed to be relevant for melanoma progression the presence of dipeptidyl peptidase IV can be used to support diagnosis of deep penetrating nevi in doubtful cases .
	manualset3
178009	6	413799	7	NULL	NULL	0	NULL	dipeptidyl peptidase IV	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results add evidence that among the selected markers supposed to be relevant for melanoma progression the presence of dipeptidyl peptidase IV can be used to support diagnosis of deep penetrating nevi in doubtful cases .
	manualset3
178010	7	413799	7	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results add evidence that among the selected markers supposed to be relevant for melanoma progression the presence of dipeptidyl peptidase IV can be used to support diagnosis of deep penetrating nevi in doubtful cases .
	manualset3
178455	8	413799	7	NULL	NULL	0	NULL	deep penetrating nevi 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results add evidence that among the selected markers supposed to be relevant for melanoma progression the presence of dipeptidyl peptidase IV can be used to support diagnosis of deep penetrating nevi in doubtful cases .
	manualset3
178456	9	413799	7	NULL	NULL	0	NULL	 cases 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results add evidence that among the selected markers supposed to be relevant for melanoma progression the presence of dipeptidyl peptidase IV can be used to support diagnosis of deep penetrating nevi in doubtful cases .
	manualset3
178457	1	413800	7	NULL	NULL	0	NULL	 results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results add swarming motility to the rapidly expanding list of phenotypes known to be controlled through quorum sensing .
	manualset3
178458	2	413800	7	NULL	NULL	0	NULL	swarming motility	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results add swarming motility to the rapidly expanding list of phenotypes known to be controlled through quorum sensing .
	manualset3
178459	3	413800	7	NULL	NULL	0	NULL	 list	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results add swarming motility to the rapidly expanding list of phenotypes known to be controlled through quorum sensing .
	manualset3
178460	4	413800	7	NULL	NULL	0	NULL	phenotypes	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results add swarming motility to the rapidly expanding list of phenotypes known to be controlled through quorum sensing .
	manualset3
178461	5	413800	7	NULL	NULL	0	NULL	quorum sensing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results add swarming motility to the rapidly expanding list of phenotypes known to be controlled through quorum sensing .
	manualset3
178462	1	413801	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results and others reported below suggest that Scutwork may play a significant role in the residency selection process .
	manualset3
178463	2	413801	7	NULL	NULL	0	NULL	Scutwork	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	These results and others reported below suggest that Scutwork may play a significant role in the residency selection process .
	manualset3
178464	3	413801	7	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results and others reported below suggest that Scutwork may play a significant role in the residency selection process .
	manualset3
178465	4	413801	7	NULL	NULL	0	NULL	residency selection process 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results and others reported below suggest that Scutwork may play a significant role in the residency selection process .
	manualset3
178466	1	413802	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are compared with the entities evidenced in dynamic light scattering measurements , the size of which is two order of magnitude higher , ca .
	manualset3
178467	2	413802	7	NULL	NULL	0	NULL	dynamic light scattering measurements	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are compared with the entities evidenced in dynamic light scattering measurements , the size of which is two order of magnitude higher , ca .
	manualset3
178468	3	413802	7	NULL	NULL	0	NULL	size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are compared with the entities evidenced in dynamic light scattering measurements , the size of which is two order of magnitude higher , ca .
	manualset3
178469	4	413802	7	NULL	NULL	0	NULL	 magnitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are compared with the entities evidenced in dynamic light scattering measurements , the size of which is two order of magnitude higher , ca .
	manualset3
178470	5	413802	7	NULL	NULL	0	NULL	ca	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are compared with the entities evidenced in dynamic light scattering measurements , the size of which is two order of magnitude higher , ca .
	manualset3
178471	6	413802	7	NULL	NULL	NULL	NULL	two order	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results are compared with the entities evidenced in dynamic light scattering measurements , the size of which is two order of magnitude higher , ca .
	manualset3
178472	7	413802	7	NULL	NULL	0	NULL	entities 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are compared with the entities evidenced in dynamic light scattering measurements , the size of which is two order of magnitude higher , ca .
	manualset3
178473	1	413803	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are compared with the principal components of the amide deuterons in solid poly ( gamma-benzyl-L-glutamate ) measured in powder samples over a wide temperature range ( 140-400 K ) .
	manualset3
178474	2	413803	7	NULL	NULL	0	NULL	principal components	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are compared with the principal components of the amide deuterons in solid poly ( gamma-benzyl-L-glutamate ) measured in powder samples over a wide temperature range ( 140-400 K ) .
	manualset3
178475	3	413803	7	NULL	NULL	0	NULL	amide deuterons	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are compared with the principal components of the amide deuterons in solid poly ( gamma-benzyl-L-glutamate ) measured in powder samples over a wide temperature range ( 140-400 K ) .
	manualset3
178476	4	413803	7	NULL	NULL	0	NULL	solid poly ( gamma-benzyl-L-glutamate )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are compared with the principal components of the amide deuterons in solid poly ( gamma-benzyl-L-glutamate ) measured in powder samples over a wide temperature range ( 140-400 K ) .
	manualset3
178477	5	413803	7	NULL	NULL	0	NULL	powder samples	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are compared with the principal components of the amide deuterons in solid poly ( gamma-benzyl-L-glutamate ) measured in powder samples over a wide temperature range ( 140-400 K ) .
	manualset3
178478	6	413803	7	NULL	NULL	0	NULL	temperature range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are compared with the principal components of the amide deuterons in solid poly ( gamma-benzyl-L-glutamate ) measured in powder samples over a wide temperature range ( 140-400 K ) .
	manualset3
178479	7	413803	7	NULL	NULL	0	NULL	140-400 K	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are compared with the principal components of the amide deuterons in solid poly ( gamma-benzyl-L-glutamate ) measured in powder samples over a wide temperature range ( 140-400 K ) .
	manualset3
178480	1	413804	7	NULL	NULL	0	NULL	nucleotide base changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional nucleotide base changes were detected among the S. falcatula isolates , but these changes were not consistent in all the S. falcatula isolates .
	manualset3
178481	2	413804	7	NULL	NULL	0	NULL	S. falcatula isolates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional nucleotide base changes were detected among the S. falcatula isolates , but these changes were not consistent in all the S. falcatula isolates .
	manualset3
178482	3	413804	7	NULL	NULL	0	NULL	changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional nucleotide base changes were detected among the S. falcatula isolates , but these changes were not consistent in all the S. falcatula isolates .
	manualset3
178483	4	413804	7	NULL	NULL	NULL	NULL	S. falcatula isolates	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Additional nucleotide base changes were detected among the S. falcatula isolates , but these changes were not consistent in all the S. falcatula isolates .
	manualset3
178484	1	413805	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with a hypothesis in which both the sinusoidal uptake of TBuMA into hepatocytes via the OCT1 and the canalicular excretion of the compound from hepatocytes via the P-gp are decreased by LPS-induced Al .
	manualset3
178485	2	413805	7	NULL	NULL	0	NULL	hypothesis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with a hypothesis in which both the sinusoidal uptake of TBuMA into hepatocytes via the OCT1 and the canalicular excretion of the compound from hepatocytes via the P-gp are decreased by LPS-induced Al .
	manualset3
178486	3	413805	7	NULL	NULL	0	NULL	sinusoidal uptake	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with a hypothesis in which both the sinusoidal uptake of TBuMA into hepatocytes via the OCT1 and the canalicular excretion of the compound from hepatocytes via the P-gp are decreased by LPS-induced Al .
	manualset3
178487	4	413805	7	NULL	NULL	0	NULL	TBuMA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with a hypothesis in which both the sinusoidal uptake of TBuMA into hepatocytes via the OCT1 and the canalicular excretion of the compound from hepatocytes via the P-gp are decreased by LPS-induced Al .
	manualset3
178488	5	413805	7	NULL	NULL	0	NULL	hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with a hypothesis in which both the sinusoidal uptake of TBuMA into hepatocytes via the OCT1 and the canalicular excretion of the compound from hepatocytes via the P-gp are decreased by LPS-induced Al .
	manualset3
178489	6	413805	7	NULL	NULL	0	NULL	 OCT1 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with a hypothesis in which both the sinusoidal uptake of TBuMA into hepatocytes via the OCT1 and the canalicular excretion of the compound from hepatocytes via the P-gp are decreased by LPS-induced Al .
	manualset3
178490	7	413805	7	NULL	NULL	0	NULL	canalicular excretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with a hypothesis in which both the sinusoidal uptake of TBuMA into hepatocytes via the OCT1 and the canalicular excretion of the compound from hepatocytes via the P-gp are decreased by LPS-induced Al .
	manualset3
178491	8	413805	7	NULL	NULL	0	NULL	compound	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with a hypothesis in which both the sinusoidal uptake of TBuMA into hepatocytes via the OCT1 and the canalicular excretion of the compound from hepatocytes via the P-gp are decreased by LPS-induced Al .
	manualset3
178492	9	413805	7	NULL	NULL	0	NULL	hepatocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with a hypothesis in which both the sinusoidal uptake of TBuMA into hepatocytes via the OCT1 and the canalicular excretion of the compound from hepatocytes via the P-gp are decreased by LPS-induced Al .
	manualset3
178493	10	413805	7	NULL	NULL	0	NULL	P-gp	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with a hypothesis in which both the sinusoidal uptake of TBuMA into hepatocytes via the OCT1 and the canalicular excretion of the compound from hepatocytes via the P-gp are decreased by LPS-induced Al .
	manualset3
178494	11	413805	7	NULL	NULL	0	NULL	LPS-induced Al	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with a hypothesis in which both the sinusoidal uptake of TBuMA into hepatocytes via the OCT1 and the canalicular excretion of the compound from hepatocytes via the P-gp are decreased by LPS-induced Al .
	manualset3
178495	1	413806	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with lumenal transmission of the DPP survival signal during imaginal disc development .
	manualset3
178496	2	413806	7	NULL	NULL	0	NULL	lumenal transmission	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with lumenal transmission of the DPP survival signal during imaginal disc development .
	manualset3
178497	3	413806	7	NULL	NULL	0	NULL	DPP survival signal	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with lumenal transmission of the DPP survival signal during imaginal disc development .
	manualset3
178498	4	413806	7	NULL	NULL	0	NULL	imaginal disc development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with lumenal transmission of the DPP survival signal during imaginal disc development .
	manualset3
178499	1	413807	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with the hypothesis that AM404 inhibits anandamide inactivation in vivo .
	manualset3
178500	2	413807	7	NULL	NULL	NULL	NULL	hypothesis	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results are consistent with the hypothesis that AM404 inhibits anandamide inactivation in vivo .
	manualset3
178501	3	413807	7	NULL	NULL	0	NULL	AM404	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with the hypothesis that AM404 inhibits anandamide inactivation in vivo .
	manualset3
178502	4	413807	7	NULL	NULL	NULL	NULL	anandamide inactivation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results are consistent with the hypothesis that AM404 inhibits anandamide inactivation in vivo .
	manualset3
178530	1	413808	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with the idea that VFA are the inhibitory substances in rumen fluid .
	manualset3
178531	2	413808	7	NULL	NULL	0	NULL	 idea	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with the idea that VFA are the inhibitory substances in rumen fluid .
	manualset3
178532	3	413808	7	NULL	NULL	0	NULL	VFA	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with the idea that VFA are the inhibitory substances in rumen fluid .
	manualset3
178533	4	413808	7	NULL	NULL	0	NULL	inhibitory substances	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with the idea that VFA are the inhibitory substances in rumen fluid .
	manualset3
178534	5	413808	7	NULL	NULL	0	NULL	rumen fluid 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with the idea that VFA are the inhibitory substances in rumen fluid .
	manualset3
178535	1	413809	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with the modifications occurring in the hepatic handling of BSP during pregnancy together with a marked impermeability of the placenta to the dye , at least in the mother-to-fetus direction .
	manualset3
178536	2	413809	7	NULL	NULL	0	NULL	modifications 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with the modifications occurring in the hepatic handling of BSP during pregnancy together with a marked impermeability of the placenta to the dye , at least in the mother-to-fetus direction .
	manualset3
178537	3	413809	7	NULL	NULL	0	NULL	BSP 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with the modifications occurring in the hepatic handling of BSP during pregnancy together with a marked impermeability of the placenta to the dye , at least in the mother-to-fetus direction .
	manualset3
178538	4	413809	7	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with the modifications occurring in the hepatic handling of BSP during pregnancy together with a marked impermeability of the placenta to the dye , at least in the mother-to-fetus direction .
	manualset3
178539	5	413809	7	NULL	NULL	0	NULL	impermeability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with the modifications occurring in the hepatic handling of BSP during pregnancy together with a marked impermeability of the placenta to the dye , at least in the mother-to-fetus direction .
	manualset3
178540	6	413809	7	NULL	NULL	0	NULL	placenta	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with the modifications occurring in the hepatic handling of BSP during pregnancy together with a marked impermeability of the placenta to the dye , at least in the mother-to-fetus direction .
	manualset3
178541	7	413809	7	NULL	NULL	0	NULL	dye	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with the modifications occurring in the hepatic handling of BSP during pregnancy together with a marked impermeability of the placenta to the dye , at least in the mother-to-fetus direction .
	manualset3
178542	8	413809	7	NULL	NULL	0	NULL	mother-to-fetus direction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with the modifications occurring in the hepatic handling of BSP during pregnancy together with a marked impermeability of the placenta to the dye , at least in the mother-to-fetus direction .
	manualset3
180345	9	413809	7	NULL	NULL	0	NULL	hepatic handling	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with the modifications occurring in the hepatic handling of BSP during pregnancy together with a marked impermeability of the placenta to the dye , at least in the mother-to-fetus direction .
	manualset3
178543	1	413810	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with transposition of Tn4351 and with insertion at several different locations in the P. gingivalis chromosome .
	manualset3
178544	2	413810	7	NULL	NULL	0	NULL	transposition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with transposition of Tn4351 and with insertion at several different locations in the P. gingivalis chromosome .
	manualset3
178545	3	413810	7	NULL	NULL	0	NULL	Tn4351	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with transposition of Tn4351 and with insertion at several different locations in the P. gingivalis chromosome .
	manualset3
178546	4	413810	7	NULL	NULL	0	NULL	 insertion 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with transposition of Tn4351 and with insertion at several different locations in the P. gingivalis chromosome .
	manualset3
178547	5	413810	7	NULL	NULL	0	NULL	different locations	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with transposition of Tn4351 and with insertion at several different locations in the P. gingivalis chromosome .
	manualset3
178548	6	413810	7	NULL	NULL	0	NULL	P. gingivalis chromosome 	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are consistent with transposition of Tn4351 and with insertion at several different locations in the P. gingivalis chromosome .
	manualset3
178625	1	413811	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are discussed in relation to proposed mechanisms for the transport of ions and water across this secretory epithelium , with particular emphasis on the role of K + as the ` prime mover ' in this process .
	manualset3
178626	2	413811	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are discussed in relation to proposed mechanisms for the transport of ions and water across this secretory epithelium , with particular emphasis on the role of K + as the ` prime mover ' in this process .
	manualset3
178627	3	413811	7	NULL	NULL	0	NULL	transport	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are discussed in relation to proposed mechanisms for the transport of ions and water across this secretory epithelium , with particular emphasis on the role of K + as the ` prime mover ' in this process .
	manualset3
178628	4	413811	7	NULL	NULL	0	NULL	 ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are discussed in relation to proposed mechanisms for the transport of ions and water across this secretory epithelium , with particular emphasis on the role of K + as the ` prime mover ' in this process .
	manualset3
178629	5	413811	7	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are discussed in relation to proposed mechanisms for the transport of ions and water across this secretory epithelium , with particular emphasis on the role of K + as the ` prime mover ' in this process .
	manualset3
178630	6	413811	7	NULL	NULL	0	NULL	secretory epithelium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are discussed in relation to proposed mechanisms for the transport of ions and water across this secretory epithelium , with particular emphasis on the role of K + as the ` prime mover ' in this process .
	manualset3
178631	7	413811	7	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are discussed in relation to proposed mechanisms for the transport of ions and water across this secretory epithelium , with particular emphasis on the role of K + as the ` prime mover ' in this process .
	manualset3
178632	8	413811	7	NULL	NULL	0	NULL	K +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are discussed in relation to proposed mechanisms for the transport of ions and water across this secretory epithelium , with particular emphasis on the role of K + as the ` prime mover ' in this process .
	manualset3
178633	9	413811	7	NULL	NULL	0	NULL	prime mover ' 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are discussed in relation to proposed mechanisms for the transport of ions and water across this secretory epithelium , with particular emphasis on the role of K + as the ` prime mover ' in this process .
	manualset3
178634	10	413811	7	NULL	NULL	0	NULL	process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are discussed in relation to proposed mechanisms for the transport of ions and water across this secretory epithelium , with particular emphasis on the role of K + as the ` prime mover ' in this process .
	manualset3
178635	11	413811	7	NULL	NULL	0	NULL	mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are discussed in relation to proposed mechanisms for the transport of ions and water across this secretory epithelium , with particular emphasis on the role of K + as the ` prime mover ' in this process .
	manualset3
178636	1	413812	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are informative for the clinical application of chondrocyte transplantation in three-dimensional cultures for cartilage repair .
	manualset3
178637	2	413812	7	NULL	NULL	0	NULL	clinical application	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are informative for the clinical application of chondrocyte transplantation in three-dimensional cultures for cartilage repair .
	manualset3
178638	3	413812	7	NULL	NULL	0	NULL	chondrocyte transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are informative for the clinical application of chondrocyte transplantation in three-dimensional cultures for cartilage repair .
	manualset3
178639	4	413812	7	NULL	NULL	0	NULL	three-dimensional cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are informative for the clinical application of chondrocyte transplantation in three-dimensional cultures for cartilage repair .
	manualset3
178640	5	413812	7	NULL	NULL	0	NULL	cartilage repair	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are informative for the clinical application of chondrocyte transplantation in three-dimensional cultures for cartilage repair .
	manualset3
178641	1	413813	7	NULL	NULL	0	NULL	Comparative study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative study of 3 algorithms to localize the accessory pathway in Wolff-Parkinson-White syndrome ) .
	manualset3
178642	2	413813	7	NULL	NULL	0	NULL	3 algorithms 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative study of 3 algorithms to localize the accessory pathway in Wolff-Parkinson-White syndrome ) .
	manualset3
178643	3	413813	7	NULL	NULL	0	NULL	accessory pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative study of 3 algorithms to localize the accessory pathway in Wolff-Parkinson-White syndrome ) .
	manualset3
178644	4	413813	7	NULL	NULL	0	NULL	Wolff-Parkinson-White syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative study of 3 algorithms to localize the accessory pathway in Wolff-Parkinson-White syndrome ) .
	manualset3
178645	1	413814	7	NULL	NULL	0	NULL	triangular-shaped segments	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional removal of triangular or crescent-shaped segments from adjacent sides of the wound prevented the cupping of the reconstructed ear .
	manualset3
178646	2	413814	7	NULL	NULL	0	NULL	crescent-shaped segments	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional removal of triangular or crescent-shaped segments from adjacent sides of the wound prevented the cupping of the reconstructed ear .
	manualset3
178647	3	413814	7	NULL	NULL	NULL	NULL	adjacent sides	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Additional removal of triangular or crescent-shaped segments from adjacent sides of the wound prevented the cupping of the reconstructed ear .
	manualset3
178648	4	413814	7	NULL	NULL	0	NULL	wound 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional removal of triangular or crescent-shaped segments from adjacent sides of the wound prevented the cupping of the reconstructed ear .
	manualset3
178649	5	413814	7	NULL	NULL	0	NULL	cupping	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional removal of triangular or crescent-shaped segments from adjacent sides of the wound prevented the cupping of the reconstructed ear .
	manualset3
178650	6	413814	7	NULL	NULL	0	NULL	reconstructed ear	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional removal of triangular or crescent-shaped segments from adjacent sides of the wound prevented the cupping of the reconstructed ear .
	manualset3
178651	1	413815	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are suggestive that fetal plasma Apo A-1 is derived solely from fetal sources and that the rate of production and/or clearance of Apo A-1 is altered during the latter third of human intrauterine development .
	manualset3
178652	2	413815	7	NULL	NULL	0	NULL	fetal plasma Apo A-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are suggestive that fetal plasma Apo A-1 is derived solely from fetal sources and that the rate of production and/or clearance of Apo A-1 is altered during the latter third of human intrauterine development .
	manualset3
178653	3	413815	7	NULL	NULL	0	NULL	fetal sources 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are suggestive that fetal plasma Apo A-1 is derived solely from fetal sources and that the rate of production and/or clearance of Apo A-1 is altered during the latter third of human intrauterine development .
	manualset3
178654	4	413815	7	NULL	NULL	NULL	NULL	 rate of production 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results are suggestive that fetal plasma Apo A-1 is derived solely from fetal sources and that the rate of production and/or clearance of Apo A-1 is altered during the latter third of human intrauterine development .
	manualset3
178655	5	413815	7	NULL	NULL	0	NULL	clearance 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are suggestive that fetal plasma Apo A-1 is derived solely from fetal sources and that the rate of production and/or clearance of Apo A-1 is altered during the latter third of human intrauterine development .
	manualset3
178656	6	413815	7	NULL	NULL	0	NULL	Apo A-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are suggestive that fetal plasma Apo A-1 is derived solely from fetal sources and that the rate of production and/or clearance of Apo A-1 is altered during the latter third of human intrauterine development .
	manualset3
178657	7	413815	7	NULL	NULL	0	NULL	 third 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are suggestive that fetal plasma Apo A-1 is derived solely from fetal sources and that the rate of production and/or clearance of Apo A-1 is altered during the latter third of human intrauterine development .
	manualset3
178658	8	413815	7	NULL	NULL	0	NULL	human intrauterine development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are suggestive that fetal plasma Apo A-1 is derived solely from fetal sources and that the rate of production and/or clearance of Apo A-1 is altered during the latter third of human intrauterine development .
	manualset3
178659	1	413816	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are the first evidence that VAP-1 is able to mediate leukocyte binding into a rejected organ .
	manualset3
178660	2	413816	7	NULL	NULL	0	NULL	 evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are the first evidence that VAP-1 is able to mediate leukocyte binding into a rejected organ .
	manualset3
178661	3	413816	7	NULL	NULL	0	NULL	VAP-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are the first evidence that VAP-1 is able to mediate leukocyte binding into a rejected organ .
	manualset3
178662	4	413816	7	NULL	NULL	0	NULL	 leukocyte binding 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are the first evidence that VAP-1 is able to mediate leukocyte binding into a rejected organ .
	manualset3
178663	5	413816	7	NULL	NULL	0	NULL	 rejected organ	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are the first evidence that VAP-1 is able to mediate leukocyte binding into a rejected organ .
	manualset3
178675	1	413817	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results argue that in the guinea pig model the presence of one of the toxins , ET or LT is sufficient for the development of the infection .
	manualset3
178676	2	413817	7	NULL	NULL	0	NULL	guinea pig model	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results argue that in the guinea pig model the presence of one of the toxins , ET or LT is sufficient for the development of the infection .
	manualset3
178677	3	413817	7	NULL	NULL	0	NULL	 presence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results argue that in the guinea pig model the presence of one of the toxins , ET or LT is sufficient for the development of the infection .
	manualset3
178678	4	413817	7	NULL	NULL	0	NULL	toxins	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results argue that in the guinea pig model the presence of one of the toxins , ET or LT is sufficient for the development of the infection .
	manualset3
178679	5	413817	7	NULL	NULL	0	NULL	ET	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results argue that in the guinea pig model the presence of one of the toxins , ET or LT is sufficient for the development of the infection .
	manualset3
178680	6	413817	7	NULL	NULL	0	NULL	LT	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results argue that in the guinea pig model the presence of one of the toxins , ET or LT is sufficient for the development of the infection .
	manualset3
178681	7	413817	7	NULL	NULL	0	NULL	development	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results argue that in the guinea pig model the presence of one of the toxins , ET or LT is sufficient for the development of the infection .
	manualset3
178682	8	413817	7	NULL	NULL	0	NULL	 infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results argue that in the guinea pig model the presence of one of the toxins , ET or LT is sufficient for the development of the infection .
	manualset3
178683	1	413818	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results as well as the histological approach suggest a correlation between expression of the aux1 and aux2 genes and cell division .
	manualset3
178684	2	413818	7	NULL	NULL	0	NULL	histological approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results as well as the histological approach suggest a correlation between expression of the aux1 and aux2 genes and cell division .
	manualset3
178685	3	413818	7	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These results as well as the histological approach suggest a correlation between expression of the aux1 and aux2 genes and cell division .
	manualset3
178686	4	413818	7	NULL	NULL	0	NULL	 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results as well as the histological approach suggest a correlation between expression of the aux1 and aux2 genes and cell division .
	manualset3
178687	5	413818	7	NULL	NULL	0	NULL	aux1 genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	These results as well as the histological approach suggest a correlation between expression of the aux1 and aux2 genes and cell division .
	manualset3
178688	6	413818	7	NULL	NULL	0	NULL	aux2 genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	These results as well as the histological approach suggest a correlation between expression of the aux1 and aux2 genes and cell division .
	manualset3
178689	7	413818	7	NULL	NULL	0	NULL	cell division	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results as well as the histological approach suggest a correlation between expression of the aux1 and aux2 genes and cell division .
	manualset3
178690	1	413819	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results both verified the head-to-head CD2-CD48 docking alignment and demonstrated the ability to elucidate the structure-function relationships of adhesion proteins from the measured distance dependence of their interaction potentials .
	manualset3
178691	2	413819	7	NULL	NULL	0	NULL	head-to-head CD2-CD48 docking alignment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results both verified the head-to-head CD2-CD48 docking alignment and demonstrated the ability to elucidate the structure-function relationships of adhesion proteins from the measured distance dependence of their interaction potentials .
	manualset3
178692	3	413819	7	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results both verified the head-to-head CD2-CD48 docking alignment and demonstrated the ability to elucidate the structure-function relationships of adhesion proteins from the measured distance dependence of their interaction potentials .
	manualset3
178693	4	413819	7	NULL	NULL	0	NULL	structure-function relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These results both verified the head-to-head CD2-CD48 docking alignment and demonstrated the ability to elucidate the structure-function relationships of adhesion proteins from the measured distance dependence of their interaction potentials .
	manualset3
178694	5	413819	7	NULL	NULL	0	NULL	adhesion proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results both verified the head-to-head CD2-CD48 docking alignment and demonstrated the ability to elucidate the structure-function relationships of adhesion proteins from the measured distance dependence of their interaction potentials .
	manualset3
178695	6	413819	7	NULL	NULL	0	NULL	measured distance	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results both verified the head-to-head CD2-CD48 docking alignment and demonstrated the ability to elucidate the structure-function relationships of adhesion proteins from the measured distance dependence of their interaction potentials .
	manualset3
178696	7	413819	7	NULL	NULL	0	NULL	interaction potentials 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results both verified the head-to-head CD2-CD48 docking alignment and demonstrated the ability to elucidate the structure-function relationships of adhesion proteins from the measured distance dependence of their interaction potentials .
	manualset3
178697	1	413820	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results can give useful insights for improving prediction methodologies which take the species specific information into account .
	manualset3
178698	2	413820	7	NULL	NULL	0	NULL	prediction methodologies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results can give useful insights for improving prediction methodologies which take the species specific information into account .
	manualset3
178699	3	413820	7	NULL	NULL	0	NULL	species specific information	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results can give useful insights for improving prediction methodologies which take the species specific information into account .
	manualset3
178700	1	413821	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results clearly demonstrated that the VZ generates relatively few precursor cells and that these oligodendrocyte precursors actively generate their cohort in the parenchyma of the CNS .
	manualset3
178701	2	413821	7	NULL	NULL	0	NULL	VZ	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results clearly demonstrated that the VZ generates relatively few precursor cells and that these oligodendrocyte precursors actively generate their cohort in the parenchyma of the CNS .
	manualset3
178702	3	413821	7	NULL	NULL	0	NULL	precursor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results clearly demonstrated that the VZ generates relatively few precursor cells and that these oligodendrocyte precursors actively generate their cohort in the parenchyma of the CNS .
	manualset3
178703	4	413821	7	NULL	NULL	0	NULL	oligodendrocyte precursors	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results clearly demonstrated that the VZ generates relatively few precursor cells and that these oligodendrocyte precursors actively generate their cohort in the parenchyma of the CNS .
	manualset3
178704	5	413821	7	NULL	NULL	0	NULL	cohort	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results clearly demonstrated that the VZ generates relatively few precursor cells and that these oligodendrocyte precursors actively generate their cohort in the parenchyma of the CNS .
	manualset3
178705	6	413821	7	NULL	NULL	0	NULL	parenchyma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results clearly demonstrated that the VZ generates relatively few precursor cells and that these oligodendrocyte precursors actively generate their cohort in the parenchyma of the CNS .
	manualset3
178706	7	413821	7	NULL	NULL	0	NULL	CNS	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results clearly demonstrated that the VZ generates relatively few precursor cells and that these oligodendrocyte precursors actively generate their cohort in the parenchyma of the CNS .
	manualset3
178731	1	413822	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results clearly suggest that 24R , 25 ( OH ) 2D3 given in massive doses has the pharmacological action of increasing bone volume in the rat without causing remarkable hypercalcemia .
	manualset3
178734	2	413822	7	NULL	NULL	0	NULL	24R , 25 ( OH ) 2D3 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results clearly suggest that 24R , 25 ( OH ) 2D3 given in massive doses has the pharmacological action of increasing bone volume in the rat without causing remarkable hypercalcemia .
	manualset3
178735	3	413822	7	NULL	NULL	0	NULL	massive doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results clearly suggest that 24R , 25 ( OH ) 2D3 given in massive doses has the pharmacological action of increasing bone volume in the rat without causing remarkable hypercalcemia .
	manualset3
178736	4	413822	7	NULL	NULL	0	NULL	pharmacological action 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results clearly suggest that 24R , 25 ( OH ) 2D3 given in massive doses has the pharmacological action of increasing bone volume in the rat without causing remarkable hypercalcemia .
	manualset3
178737	5	413822	7	NULL	NULL	0	NULL	bone volume 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results clearly suggest that 24R , 25 ( OH ) 2D3 given in massive doses has the pharmacological action of increasing bone volume in the rat without causing remarkable hypercalcemia .
	manualset3
178738	6	413822	7	NULL	NULL	0	NULL	rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results clearly suggest that 24R , 25 ( OH ) 2D3 given in massive doses has the pharmacological action of increasing bone volume in the rat without causing remarkable hypercalcemia .
	manualset3
178739	7	413822	7	NULL	NULL	0	NULL	hypercalcemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results clearly suggest that 24R , 25 ( OH ) 2D3 given in massive doses has the pharmacological action of increasing bone volume in the rat without causing remarkable hypercalcemia .
	manualset3
178740	1	413823	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results confirm that Ca ( 2 + ) inhibits elimination of H ( 2 ) O ( 2 ) in mitochondria and demonstrate that this effect is concentration dependent and reversible .
	manualset3
178741	2	413823	7	NULL	NULL	0	NULL	Ca ( 2 + )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	These results confirm that Ca ( 2 + ) inhibits elimination of H ( 2 ) O ( 2 ) in mitochondria and demonstrate that this effect is concentration dependent and reversible .
	manualset3
178742	3	413823	7	NULL	NULL	0	NULL	elimination 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results confirm that Ca ( 2 + ) inhibits elimination of H ( 2 ) O ( 2 ) in mitochondria and demonstrate that this effect is concentration dependent and reversible .
	manualset3
178743	4	413823	7	NULL	NULL	0	NULL	H ( 2 ) O ( 2 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results confirm that Ca ( 2 + ) inhibits elimination of H ( 2 ) O ( 2 ) in mitochondria and demonstrate that this effect is concentration dependent and reversible .
	manualset3
178744	5	413823	7	NULL	NULL	0	NULL	mitochondria	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These results confirm that Ca ( 2 + ) inhibits elimination of H ( 2 ) O ( 2 ) in mitochondria and demonstrate that this effect is concentration dependent and reversible .
	manualset3
178745	6	413823	7	NULL	NULL	0	NULL	effect 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results confirm that Ca ( 2 + ) inhibits elimination of H ( 2 ) O ( 2 ) in mitochondria and demonstrate that this effect is concentration dependent and reversible .
	manualset3
178746	7	413823	7	NULL	NULL	0	NULL	concentration dependent	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results confirm that Ca ( 2 + ) inhibits elimination of H ( 2 ) O ( 2 ) in mitochondria and demonstrate that this effect is concentration dependent and reversible .
	manualset3
178747	1	413824	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results confirm that in high agricultural activity areas , A. funestus can be by far the major malaria vector responsible for malaria transmission .
	manualset3
178748	2	413824	7	NULL	NULL	0	NULL	high agricultural activity areas	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	These results confirm that in high agricultural activity areas , A. funestus can be by far the major malaria vector responsible for malaria transmission .
	manualset3
178749	3	413824	7	NULL	NULL	0	NULL	A. funestus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results confirm that in high agricultural activity areas , A. funestus can be by far the major malaria vector responsible for malaria transmission .
	manualset3
178750	4	413824	7	NULL	NULL	0	NULL	malaria vector	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results confirm that in high agricultural activity areas , A. funestus can be by far the major malaria vector responsible for malaria transmission .
	manualset3
178751	5	413824	7	NULL	NULL	0	NULL	malaria transmission	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results confirm that in high agricultural activity areas , A. funestus can be by far the major malaria vector responsible for malaria transmission .
	manualset3
178752	1	413825	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results confirm that spoligotyping and VNTR analysis are valuable tools for studying the molecular epidemiology of M. bovis infections in Brazil .
	manualset3
178753	2	413825	7	NULL	NULL	0	NULL	spoligotyping	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results confirm that spoligotyping and VNTR analysis are valuable tools for studying the molecular epidemiology of M. bovis infections in Brazil .
	manualset3
178754	3	413825	7	NULL	NULL	0	NULL	VNTR analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results confirm that spoligotyping and VNTR analysis are valuable tools for studying the molecular epidemiology of M. bovis infections in Brazil .
	manualset3
178755	4	413825	7	NULL	NULL	0	NULL	tools	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These results confirm that spoligotyping and VNTR analysis are valuable tools for studying the molecular epidemiology of M. bovis infections in Brazil .
	manualset3
178758	5	413825	7	NULL	NULL	0	NULL	molecular epidemiology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These results confirm that spoligotyping and VNTR analysis are valuable tools for studying the molecular epidemiology of M. bovis infections in Brazil .
	manualset3
178759	7	413825	7	NULL	NULL	NULL	NULL	Brazil	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results confirm that spoligotyping and VNTR analysis are valuable tools for studying the molecular epidemiology of M. bovis infections in Brazil .
	manualset3
178844	6	413825	7	NULL	NULL	0	NULL	M. bovis infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results confirm that spoligotyping and VNTR analysis are valuable tools for studying the molecular epidemiology of M. bovis infections in Brazil .
	manualset3
178845	1	413826	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate for the first time distinct conformational determinants characteristic of activating versus tolerogenic MHC-peptide complexes involved in human autoimmunity .
	manualset3
178846	2	413826	7	NULL	NULL	0	NULL	first time	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate for the first time distinct conformational determinants characteristic of activating versus tolerogenic MHC-peptide complexes involved in human autoimmunity .
	manualset3
178847	3	413826	7	NULL	NULL	0	NULL	conformational determinants	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate for the first time distinct conformational determinants characteristic of activating versus tolerogenic MHC-peptide complexes involved in human autoimmunity .
	manualset3
178848	4	413826	7	NULL	NULL	NULL	NULL	tolerogenic MHC-peptide complexes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results demonstrate for the first time distinct conformational determinants characteristic of activating versus tolerogenic MHC-peptide complexes involved in human autoimmunity .
	manualset3
178849	5	413826	7	NULL	NULL	0	NULL	human autoimmunity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate for the first time distinct conformational determinants characteristic of activating versus tolerogenic MHC-peptide complexes involved in human autoimmunity .
	manualset3
178850	1	413827	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that ( 1 ) skeletal muscle plays an important role in the metabolism of dietary ethanol , ( 2 ) the fed state appears to favor the conversion of ethanol-derived carbons to lipid , and ( 3 ) female rats have a greater propensity to convert ethanol-derived carbons to lipid and to store these carbons in adipose tissue .
	manualset3
178851	2	413827	7	NULL	NULL	0	NULL	skeletal muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that ( 1 ) skeletal muscle plays an important role in the metabolism of dietary ethanol , ( 2 ) the fed state appears to favor the conversion of ethanol-derived carbons to lipid , and ( 3 ) female rats have a greater propensity to convert ethanol-derived carbons to lipid and to store these carbons in adipose tissue .
	manualset3
178852	3	413827	7	NULL	NULL	NULL	NULL	role	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results demonstrate that ( 1 ) skeletal muscle plays an important role in the metabolism of dietary ethanol , ( 2 ) the fed state appears to favor the conversion of ethanol-derived carbons to lipid , and ( 3 ) female rats have a greater propensity to convert ethanol-derived carbons to lipid and to store these carbons in adipose tissue .
	manualset3
178853	4	413827	7	NULL	NULL	NULL	NULL	 metabolism 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results demonstrate that ( 1 ) skeletal muscle plays an important role in the metabolism of dietary ethanol , ( 2 ) the fed state appears to favor the conversion of ethanol-derived carbons to lipid , and ( 3 ) female rats have a greater propensity to convert ethanol-derived carbons to lipid and to store these carbons in adipose tissue .
	manualset3
178854	5	413827	7	NULL	NULL	0	NULL	dietary ethanol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that ( 1 ) skeletal muscle plays an important role in the metabolism of dietary ethanol , ( 2 ) the fed state appears to favor the conversion of ethanol-derived carbons to lipid , and ( 3 ) female rats have a greater propensity to convert ethanol-derived carbons to lipid and to store these carbons in adipose tissue .
	manualset3
178855	6	413827	7	NULL	NULL	0	NULL	fed state 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that ( 1 ) skeletal muscle plays an important role in the metabolism of dietary ethanol , ( 2 ) the fed state appears to favor the conversion of ethanol-derived carbons to lipid , and ( 3 ) female rats have a greater propensity to convert ethanol-derived carbons to lipid and to store these carbons in adipose tissue .
	manualset3
178856	7	413827	7	NULL	NULL	0	NULL	conversion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that ( 1 ) skeletal muscle plays an important role in the metabolism of dietary ethanol , ( 2 ) the fed state appears to favor the conversion of ethanol-derived carbons to lipid , and ( 3 ) female rats have a greater propensity to convert ethanol-derived carbons to lipid and to store these carbons in adipose tissue .
	manualset3
178857	8	413827	7	NULL	NULL	0	NULL	ethanol-derived carbons 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that ( 1 ) skeletal muscle plays an important role in the metabolism of dietary ethanol , ( 2 ) the fed state appears to favor the conversion of ethanol-derived carbons to lipid , and ( 3 ) female rats have a greater propensity to convert ethanol-derived carbons to lipid and to store these carbons in adipose tissue .
	manualset3
178858	9	413827	7	NULL	NULL	NULL	NULL	lipid	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results demonstrate that ( 1 ) skeletal muscle plays an important role in the metabolism of dietary ethanol , ( 2 ) the fed state appears to favor the conversion of ethanol-derived carbons to lipid , and ( 3 ) female rats have a greater propensity to convert ethanol-derived carbons to lipid and to store these carbons in adipose tissue .
	manualset3
178859	10	413827	7	NULL	NULL	0	NULL	 female rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that ( 1 ) skeletal muscle plays an important role in the metabolism of dietary ethanol , ( 2 ) the fed state appears to favor the conversion of ethanol-derived carbons to lipid , and ( 3 ) female rats have a greater propensity to convert ethanol-derived carbons to lipid and to store these carbons in adipose tissue .
	manualset3
178860	11	413827	7	NULL	NULL	0	NULL	propensity 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that ( 1 ) skeletal muscle plays an important role in the metabolism of dietary ethanol , ( 2 ) the fed state appears to favor the conversion of ethanol-derived carbons to lipid , and ( 3 ) female rats have a greater propensity to convert ethanol-derived carbons to lipid and to store these carbons in adipose tissue .
	manualset3
178861	12	413827	7	NULL	NULL	0	NULL	ethanol-derived carbons	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that ( 1 ) skeletal muscle plays an important role in the metabolism of dietary ethanol , ( 2 ) the fed state appears to favor the conversion of ethanol-derived carbons to lipid , and ( 3 ) female rats have a greater propensity to convert ethanol-derived carbons to lipid and to store these carbons in adipose tissue .
	manualset3
178862	13	413827	7	NULL	NULL	NULL	NULL	lipid 	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results demonstrate that ( 1 ) skeletal muscle plays an important role in the metabolism of dietary ethanol , ( 2 ) the fed state appears to favor the conversion of ethanol-derived carbons to lipid , and ( 3 ) female rats have a greater propensity to convert ethanol-derived carbons to lipid and to store these carbons in adipose tissue .
	manualset3
178863	14	413827	7	NULL	NULL	0	NULL	carbons	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that ( 1 ) skeletal muscle plays an important role in the metabolism of dietary ethanol , ( 2 ) the fed state appears to favor the conversion of ethanol-derived carbons to lipid , and ( 3 ) female rats have a greater propensity to convert ethanol-derived carbons to lipid and to store these carbons in adipose tissue .
	manualset3
178864	15	413827	7	NULL	NULL	0	NULL	adipose tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that ( 1 ) skeletal muscle plays an important role in the metabolism of dietary ethanol , ( 2 ) the fed state appears to favor the conversion of ethanol-derived carbons to lipid , and ( 3 ) female rats have a greater propensity to convert ethanol-derived carbons to lipid and to store these carbons in adipose tissue .
	manualset3
178865	1	413828	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that ISPCR is a highly sensitive method for amplifying genomic DNA sequences within intact single cells .
	manualset3
178866	2	413828	7	NULL	NULL	0	NULL	ISPCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that ISPCR is a highly sensitive method for amplifying genomic DNA sequences within intact single cells .
	manualset3
178867	3	413828	7	NULL	NULL	0	NULL	highly sensitive method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that ISPCR is a highly sensitive method for amplifying genomic DNA sequences within intact single cells .
	manualset3
178868	4	413828	7	NULL	NULL	0	NULL	genomic DNA sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that ISPCR is a highly sensitive method for amplifying genomic DNA sequences within intact single cells .
	manualset3
178869	5	413828	7	NULL	NULL	0	NULL	single cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that ISPCR is a highly sensitive method for amplifying genomic DNA sequences within intact single cells .
	manualset3
178870	1	413829	7	NULL	NULL	0	NULL	 results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that LDL , but not HDL , increases intracellular concentrations of c-myc in two different aortic smooth muscle cell lines .
	manualset3
178871	2	413829	7	NULL	NULL	0	NULL	LDL	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that LDL , but not HDL , increases intracellular concentrations of c-myc in two different aortic smooth muscle cell lines .
	manualset3
178872	3	413829	7	NULL	NULL	0	NULL	HDL	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that LDL , but not HDL , increases intracellular concentrations of c-myc in two different aortic smooth muscle cell lines .
	manualset3
178873	4	413829	7	NULL	NULL	0	NULL	intracellular concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that LDL , but not HDL , increases intracellular concentrations of c-myc in two different aortic smooth muscle cell lines .
	manualset3
178874	5	413829	7	NULL	NULL	0	NULL	c-myc	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that LDL , but not HDL , increases intracellular concentrations of c-myc in two different aortic smooth muscle cell lines .
	manualset3
178875	6	413829	7	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that LDL , but not HDL , increases intracellular concentrations of c-myc in two different aortic smooth muscle cell lines .
	manualset3
178876	7	413829	7	NULL	NULL	0	NULL	aortic smooth muscle cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that LDL , but not HDL , increases intracellular concentrations of c-myc in two different aortic smooth muscle cell lines .
	manualset3
178877	1	413830	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that a diet enriched with different FAs has strong effects on serum lipid levels and the deposition of PUFAs into tissue lipids .
	manualset3
178878	2	413830	7	NULL	NULL	0	NULL	diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that a diet enriched with different FAs has strong effects on serum lipid levels and the deposition of PUFAs into tissue lipids .
	manualset3
178879	3	413830	7	NULL	NULL	0	NULL	different FAs	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that a diet enriched with different FAs has strong effects on serum lipid levels and the deposition of PUFAs into tissue lipids .
	manualset3
178880	4	413830	7	NULL	NULL	0	NULL	strong effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that a diet enriched with different FAs has strong effects on serum lipid levels and the deposition of PUFAs into tissue lipids .
	manualset3
178881	5	413830	7	NULL	NULL	0	NULL	serum lipid levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that a diet enriched with different FAs has strong effects on serum lipid levels and the deposition of PUFAs into tissue lipids .
	manualset3
178882	6	413830	7	NULL	NULL	0	NULL	deposition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that a diet enriched with different FAs has strong effects on serum lipid levels and the deposition of PUFAs into tissue lipids .
	manualset3
178883	7	413830	7	NULL	NULL	0	NULL	PUFAs	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that a diet enriched with different FAs has strong effects on serum lipid levels and the deposition of PUFAs into tissue lipids .
	manualset3
178884	8	413830	7	NULL	NULL	0	NULL	tissue lipids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that a diet enriched with different FAs has strong effects on serum lipid levels and the deposition of PUFAs into tissue lipids .
	manualset3
178894	1	413831	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that human placenta expresses both apoB and MTP and consequently synthesize and secrete apoB-100-containing lipoproteins .
	manualset3
178895	2	413831	7	NULL	NULL	0	NULL	 human placenta	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that human placenta expresses both apoB and MTP and consequently synthesize and secrete apoB-100-containing lipoproteins .
	manualset3
178896	3	413831	7	NULL	NULL	0	NULL	apoB	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that human placenta expresses both apoB and MTP and consequently synthesize and secrete apoB-100-containing lipoproteins .
	manualset3
178897	4	413831	7	NULL	NULL	0	NULL	MTP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that human placenta expresses both apoB and MTP and consequently synthesize and secrete apoB-100-containing lipoproteins .
	manualset3
178898	5	413831	7	NULL	NULL	NULL	NULL	apoB-100-containing lipoproteins 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results demonstrate that human placenta expresses both apoB and MTP and consequently synthesize and secrete apoB-100-containing lipoproteins .
	manualset3
178899	1	413832	7	NULL	NULL	0	NULL	properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional reported properties of this inhibitor include inhibition of protein tyrosine phosphatases , nucleases and members of the Jak family .
	manualset3
178900	2	413832	7	NULL	NULL	0	NULL	inhibitor	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional reported properties of this inhibitor include inhibition of protein tyrosine phosphatases , nucleases and members of the Jak family .
	manualset3
178901	3	413832	7	NULL	NULL	0	NULL	inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional reported properties of this inhibitor include inhibition of protein tyrosine phosphatases , nucleases and members of the Jak family .
	manualset3
178902	4	413832	7	NULL	NULL	0	NULL	protein tyrosine phosphatases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional reported properties of this inhibitor include inhibition of protein tyrosine phosphatases , nucleases and members of the Jak family .
	manualset3
178903	5	413832	7	NULL	NULL	0	NULL	nucleases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional reported properties of this inhibitor include inhibition of protein tyrosine phosphatases , nucleases and members of the Jak family .
	manualset3
178904	6	413832	7	NULL	NULL	0	NULL	members	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional reported properties of this inhibitor include inhibition of protein tyrosine phosphatases , nucleases and members of the Jak family .
	manualset3
178905	7	413832	7	NULL	NULL	0	NULL	Jak family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional reported properties of this inhibitor include inhibition of protein tyrosine phosphatases , nucleases and members of the Jak family .
	manualset3
178906	1	413833	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that inhibition of the synthesis of endogenous NO may also have an inhibitory effect on the activity of sGC .
	manualset3
178907	2	413833	7	NULL	NULL	0	NULL	 inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that inhibition of the synthesis of endogenous NO may also have an inhibitory effect on the activity of sGC .
	manualset3
178908	3	413833	7	NULL	NULL	0	NULL	synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that inhibition of the synthesis of endogenous NO may also have an inhibitory effect on the activity of sGC .
	manualset3
178909	4	413833	7	NULL	NULL	0	NULL	endogenous NO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that inhibition of the synthesis of endogenous NO may also have an inhibitory effect on the activity of sGC .
	manualset3
178910	5	413833	7	NULL	NULL	0	NULL	inhibitory effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that inhibition of the synthesis of endogenous NO may also have an inhibitory effect on the activity of sGC .
	manualset3
178911	6	413833	7	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that inhibition of the synthesis of endogenous NO may also have an inhibitory effect on the activity of sGC .
	manualset3
178912	7	413833	7	NULL	NULL	0	NULL	sGC	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that inhibition of the synthesis of endogenous NO may also have an inhibitory effect on the activity of sGC .
	manualset3
178913	1	413834	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that oral viridans streptococci , probably by engaging two cell surface adhesins , exert immunomodulatory effects on human KB and endothelial cells .
	manualset3
178914	2	413834	7	NULL	NULL	0	NULL	oral viridans streptococci	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that oral viridans streptococci , probably by engaging two cell surface adhesins , exert immunomodulatory effects on human KB and endothelial cells .
	manualset3
178915	3	413834	7	NULL	NULL	0	NULL	two cell surface adhesins	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that oral viridans streptococci , probably by engaging two cell surface adhesins , exert immunomodulatory effects on human KB and endothelial cells .
	manualset3
178916	4	413834	7	NULL	NULL	0	NULL	immunomodulatory effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that oral viridans streptococci , probably by engaging two cell surface adhesins , exert immunomodulatory effects on human KB and endothelial cells .
	manualset3
178917	5	413834	7	NULL	NULL	0	NULL	human KB cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that oral viridans streptococci , probably by engaging two cell surface adhesins , exert immunomodulatory effects on human KB and endothelial cells .
	manualset3
178918	6	413834	7	NULL	NULL	0	NULL	endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that oral viridans streptococci , probably by engaging two cell surface adhesins , exert immunomodulatory effects on human KB and endothelial cells .
	manualset3
178919	1	413835	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that patients with cerebral ischemia have abnormal hemostatic function that is not explained by the acute phase reaction , and that components of the prethrombotic state are present in some of these patients .
	manualset3
178920	2	413835	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that patients with cerebral ischemia have abnormal hemostatic function that is not explained by the acute phase reaction , and that components of the prethrombotic state are present in some of these patients .
	manualset3
178921	3	413835	7	NULL	NULL	0	NULL	cerebral ischemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that patients with cerebral ischemia have abnormal hemostatic function that is not explained by the acute phase reaction , and that components of the prethrombotic state are present in some of these patients .
	manualset3
178922	4	413835	7	NULL	NULL	0	NULL	abnormal hemostatic function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that patients with cerebral ischemia have abnormal hemostatic function that is not explained by the acute phase reaction , and that components of the prethrombotic state are present in some of these patients .
	manualset3
178923	5	413835	7	NULL	NULL	0	NULL	acute phase reaction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that patients with cerebral ischemia have abnormal hemostatic function that is not explained by the acute phase reaction , and that components of the prethrombotic state are present in some of these patients .
	manualset3
178924	6	413835	7	NULL	NULL	0	NULL	components	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that patients with cerebral ischemia have abnormal hemostatic function that is not explained by the acute phase reaction , and that components of the prethrombotic state are present in some of these patients .
	manualset3
178925	7	413835	7	NULL	NULL	0	NULL	prethrombotic state	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that patients with cerebral ischemia have abnormal hemostatic function that is not explained by the acute phase reaction , and that components of the prethrombotic state are present in some of these patients .
	manualset3
178926	8	413835	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that patients with cerebral ischemia have abnormal hemostatic function that is not explained by the acute phase reaction , and that components of the prethrombotic state are present in some of these patients .
	manualset3
178927	1	413836	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that phenolic compounds have a significant contribution to the total antioxidant activity which varies considerably depending of the part of the fruit and of the apple cultivar analyzed .
	manualset3
178928	2	413836	7	NULL	NULL	0	NULL	phenolic compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that phenolic compounds have a significant contribution to the total antioxidant activity which varies considerably depending of the part of the fruit and of the apple cultivar analyzed .
	manualset3
178929	3	413836	7	NULL	NULL	0	NULL	contribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that phenolic compounds have a significant contribution to the total antioxidant activity which varies considerably depending of the part of the fruit and of the apple cultivar analyzed .
	manualset3
178930	4	413836	7	NULL	NULL	0	NULL	total antioxidant activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that phenolic compounds have a significant contribution to the total antioxidant activity which varies considerably depending of the part of the fruit and of the apple cultivar analyzed .
	manualset3
178931	5	413836	7	NULL	NULL	0	NULL	part of the fruit	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that phenolic compounds have a significant contribution to the total antioxidant activity which varies considerably depending of the part of the fruit and of the apple cultivar analyzed .
	manualset3
178932	6	413836	7	NULL	NULL	0	NULL	apple cultivar	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that phenolic compounds have a significant contribution to the total antioxidant activity which varies considerably depending of the part of the fruit and of the apple cultivar analyzed .
	manualset3
178933	1	413837	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that the methodological base of the NHP has yet to be established .
	manualset3
178934	2	413837	7	NULL	NULL	0	NULL	methodological base	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that the methodological base of the NHP has yet to be established .
	manualset3
178935	3	413837	7	NULL	NULL	0	NULL	NHP	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that the methodological base of the NHP has yet to be established .
	manualset3
178942	1	413838	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that tissue levels of LPS increase throughout the course of acute GVHD and are sufficient to trigger the release of pathologic amounts of TNF-alpha from primed macrophages resulting in the cachexia and mortality associated with acute GVHD in this model .
	manualset3
178943	2	413838	7	NULL	NULL	0	NULL	tissue levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that tissue levels of LPS increase throughout the course of acute GVHD and are sufficient to trigger the release of pathologic amounts of TNF-alpha from primed macrophages resulting in the cachexia and mortality associated with acute GVHD in this model .
	manualset3
178944	3	413838	7	NULL	NULL	0	NULL	LPS	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that tissue levels of LPS increase throughout the course of acute GVHD and are sufficient to trigger the release of pathologic amounts of TNF-alpha from primed macrophages resulting in the cachexia and mortality associated with acute GVHD in this model .
	manualset3
178945	4	413838	7	NULL	NULL	0	NULL	course	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that tissue levels of LPS increase throughout the course of acute GVHD and are sufficient to trigger the release of pathologic amounts of TNF-alpha from primed macrophages resulting in the cachexia and mortality associated with acute GVHD in this model .
	manualset3
178946	5	413838	7	NULL	NULL	0	NULL	acute GVHD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that tissue levels of LPS increase throughout the course of acute GVHD and are sufficient to trigger the release of pathologic amounts of TNF-alpha from primed macrophages resulting in the cachexia and mortality associated with acute GVHD in this model .
	manualset3
178974	6	413838	7	NULL	NULL	0	NULL	 release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that tissue levels of LPS increase throughout the course of acute GVHD and are sufficient to trigger the release of pathologic amounts of TNF-alpha from primed macrophages resulting in the cachexia and mortality associated with acute GVHD in this model .
	manualset3
178975	7	413838	7	NULL	NULL	0	NULL	pathologic amounts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that tissue levels of LPS increase throughout the course of acute GVHD and are sufficient to trigger the release of pathologic amounts of TNF-alpha from primed macrophages resulting in the cachexia and mortality associated with acute GVHD in this model .
	manualset3
178976	8	413838	7	NULL	NULL	0	NULL	TNF-alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that tissue levels of LPS increase throughout the course of acute GVHD and are sufficient to trigger the release of pathologic amounts of TNF-alpha from primed macrophages resulting in the cachexia and mortality associated with acute GVHD in this model .
	manualset3
178977	9	413838	7	NULL	NULL	0	NULL	primed macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that tissue levels of LPS increase throughout the course of acute GVHD and are sufficient to trigger the release of pathologic amounts of TNF-alpha from primed macrophages resulting in the cachexia and mortality associated with acute GVHD in this model .
	manualset3
178979	10	413838	7	NULL	NULL	0	NULL	cachexia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that tissue levels of LPS increase throughout the course of acute GVHD and are sufficient to trigger the release of pathologic amounts of TNF-alpha from primed macrophages resulting in the cachexia and mortality associated with acute GVHD in this model .
	manualset3
178980	11	413838	7	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that tissue levels of LPS increase throughout the course of acute GVHD and are sufficient to trigger the release of pathologic amounts of TNF-alpha from primed macrophages resulting in the cachexia and mortality associated with acute GVHD in this model .
	manualset3
178981	12	413838	7	NULL	NULL	0	NULL	acute GVHD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that tissue levels of LPS increase throughout the course of acute GVHD and are sufficient to trigger the release of pathologic amounts of TNF-alpha from primed macrophages resulting in the cachexia and mortality associated with acute GVHD in this model .
	manualset3
178982	13	413838	7	NULL	NULL	0	NULL	model 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate that tissue levels of LPS increase throughout the course of acute GVHD and are sufficient to trigger the release of pathologic amounts of TNF-alpha from primed macrophages resulting in the cachexia and mortality associated with acute GVHD in this model .
	manualset3
178987	1	413839	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate uptake of adenosine from both the tubular and vascular compartments , and analysis of single-injection multiple-indicator curves indicates that a substantial amount of the extracted arterial adenosine enters and remains in cells .
	manualset3
178988	2	413839	7	NULL	NULL	NULL	NULL	adenosine	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results demonstrate uptake of adenosine from both the tubular and vascular compartments , and analysis of single-injection multiple-indicator curves indicates that a substantial amount of the extracted arterial adenosine enters and remains in cells .
	manualset3
178989	3	413839	7	NULL	NULL	0	NULL	tubular compartment	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate uptake of adenosine from both the tubular and vascular compartments , and analysis of single-injection multiple-indicator curves indicates that a substantial amount of the extracted arterial adenosine enters and remains in cells .
	manualset3
178990	4	413839	7	NULL	NULL	0	NULL	vascular compartments	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate uptake of adenosine from both the tubular and vascular compartments , and analysis of single-injection multiple-indicator curves indicates that a substantial amount of the extracted arterial adenosine enters and remains in cells .
	manualset3
178991	5	413839	7	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate uptake of adenosine from both the tubular and vascular compartments , and analysis of single-injection multiple-indicator curves indicates that a substantial amount of the extracted arterial adenosine enters and remains in cells .
	manualset3
178992	6	413839	7	NULL	NULL	0	NULL	single-injection multiple-indicator curves	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate uptake of adenosine from both the tubular and vascular compartments , and analysis of single-injection multiple-indicator curves indicates that a substantial amount of the extracted arterial adenosine enters and remains in cells .
	manualset3
178993	7	413839	7	NULL	NULL	0	NULL	substantial amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate uptake of adenosine from both the tubular and vascular compartments , and analysis of single-injection multiple-indicator curves indicates that a substantial amount of the extracted arterial adenosine enters and remains in cells .
	manualset3
178994	8	413839	7	NULL	NULL	0	NULL	extracted arterial adenosine	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate uptake of adenosine from both the tubular and vascular compartments , and analysis of single-injection multiple-indicator curves indicates that a substantial amount of the extracted arterial adenosine enters and remains in cells .
	manualset3
178995	9	413839	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrate uptake of adenosine from both the tubular and vascular compartments , and analysis of single-injection multiple-indicator curves indicates that a substantial amount of the extracted arterial adenosine enters and remains in cells .
	manualset3
178999	1	413840	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrated that heart extract obtained from hypertrophied LV of perinephritic hypertensive dogs contained at least one factor which may induce and/or modulate myocardial hypertrophy in this model for hypertension .
	manualset3
179000	2	413840	7	NULL	NULL	0	NULL	heart extract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrated that heart extract obtained from hypertrophied LV of perinephritic hypertensive dogs contained at least one factor which may induce and/or modulate myocardial hypertrophy in this model for hypertension .
	manualset3
179001	3	413840	7	NULL	NULL	0	NULL	hypertrophied LV of perinephritic hypertensive dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrated that heart extract obtained from hypertrophied LV of perinephritic hypertensive dogs contained at least one factor which may induce and/or modulate myocardial hypertrophy in this model for hypertension .
	manualset3
179002	4	413840	7	NULL	NULL	0	NULL	one factor	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrated that heart extract obtained from hypertrophied LV of perinephritic hypertensive dogs contained at least one factor which may induce and/or modulate myocardial hypertrophy in this model for hypertension .
	manualset3
179003	5	413840	7	NULL	NULL	0	NULL	myocardial hypertrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrated that heart extract obtained from hypertrophied LV of perinephritic hypertensive dogs contained at least one factor which may induce and/or modulate myocardial hypertrophy in this model for hypertension .
	manualset3
179004	6	413840	7	NULL	NULL	0	NULL	model	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrated that heart extract obtained from hypertrophied LV of perinephritic hypertensive dogs contained at least one factor which may induce and/or modulate myocardial hypertrophy in this model for hypertension .
	manualset3
179005	7	413840	7	NULL	NULL	0	NULL	hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results demonstrated that heart extract obtained from hypertrophied LV of perinephritic hypertensive dogs contained at least one factor which may induce and/or modulate myocardial hypertrophy in this model for hypertension .
	manualset3
179006	1	413841	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results do not support the hypothesis that the hypotensive actions of losartan are entirely dependent on a responsive sympathetic nervous system rats .
	manualset3
179007	2	413841	7	NULL	NULL	0	NULL	hypothesis 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These results do not support the hypothesis that the hypotensive actions of losartan are entirely dependent on a responsive sympathetic nervous system rats .
	manualset3
179008	3	413841	7	NULL	NULL	0	NULL	hypotensive actions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results do not support the hypothesis that the hypotensive actions of losartan are entirely dependent on a responsive sympathetic nervous system rats .
	manualset3
179009	4	413841	7	NULL	NULL	0	NULL	losartan	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These results do not support the hypothesis that the hypotensive actions of losartan are entirely dependent on a responsive sympathetic nervous system rats .
	manualset3
179010	5	413841	7	NULL	NULL	0	NULL	sympathetic nervous system 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results do not support the hypothesis that the hypotensive actions of losartan are entirely dependent on a responsive sympathetic nervous system rats .
	manualset3
179011	6	413841	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results do not support the hypothesis that the hypotensive actions of losartan are entirely dependent on a responsive sympathetic nervous system rats .
	manualset3
179012	1	413842	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results emphasize a crucial function for Blimp-1 in controlling T cell homeostasis and activation .
	manualset3
179013	2	413842	7	NULL	NULL	0	NULL	crucial function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results emphasize a crucial function for Blimp-1 in controlling T cell homeostasis and activation .
	manualset3
179014	3	413842	7	NULL	NULL	0	NULL	Blimp-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results emphasize a crucial function for Blimp-1 in controlling T cell homeostasis and activation .
	manualset3
179015	4	413842	7	NULL	NULL	0	NULL	T cell homeostasis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results emphasize a crucial function for Blimp-1 in controlling T cell homeostasis and activation .
	manualset3
179016	5	413842	7	NULL	NULL	0	NULL	T cell activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results emphasize a crucial function for Blimp-1 in controlling T cell homeostasis and activation .
	manualset3
179017	1	413843	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results establish a pivotal role for CXCL12 signaling in HPV-mediated transformation and provide a mechanistic basis for understanding HPV pathogenesis in WHIM syndrome .
	manualset3
179018	2	413843	7	NULL	NULL	0	NULL	pivotal role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results establish a pivotal role for CXCL12 signaling in HPV-mediated transformation and provide a mechanistic basis for understanding HPV pathogenesis in WHIM syndrome .
	manualset3
179019	3	413843	7	NULL	NULL	0	NULL	CXCL12 signaling 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results establish a pivotal role for CXCL12 signaling in HPV-mediated transformation and provide a mechanistic basis for understanding HPV pathogenesis in WHIM syndrome .
	manualset3
179020	4	413843	7	NULL	NULL	0	NULL	HPV-mediated transformation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results establish a pivotal role for CXCL12 signaling in HPV-mediated transformation and provide a mechanistic basis for understanding HPV pathogenesis in WHIM syndrome .
	manualset3
179021	5	413843	7	NULL	NULL	NULL	NULL	mechanistic basis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results establish a pivotal role for CXCL12 signaling in HPV-mediated transformation and provide a mechanistic basis for understanding HPV pathogenesis in WHIM syndrome .
	manualset3
179022	6	413843	7	NULL	NULL	0	NULL	HPV pathogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results establish a pivotal role for CXCL12 signaling in HPV-mediated transformation and provide a mechanistic basis for understanding HPV pathogenesis in WHIM syndrome .
	manualset3
179023	7	413843	7	NULL	NULL	0	NULL	WHIM syndrome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results establish a pivotal role for CXCL12 signaling in HPV-mediated transformation and provide a mechanistic basis for understanding HPV pathogenesis in WHIM syndrome .
	manualset3
179025	1	413844	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results extend the computational learning approach from striatum to amygdala , demonstrating their complementary roles in aversive learning .
	manualset3
179026	2	413844	7	NULL	NULL	0	NULL	computational learning approach	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These results extend the computational learning approach from striatum to amygdala , demonstrating their complementary roles in aversive learning .
	manualset3
179027	3	413844	7	NULL	NULL	0	NULL	striatum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results extend the computational learning approach from striatum to amygdala , demonstrating their complementary roles in aversive learning .
	manualset3
179028	4	413844	7	NULL	NULL	0	NULL	amygdala	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results extend the computational learning approach from striatum to amygdala , demonstrating their complementary roles in aversive learning .
	manualset3
179029	5	413844	7	NULL	NULL	0	NULL	complementary roles	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results extend the computational learning approach from striatum to amygdala , demonstrating their complementary roles in aversive learning .
	manualset3
179030	6	413844	7	NULL	NULL	0	NULL	aversive learning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results extend the computational learning approach from striatum to amygdala , demonstrating their complementary roles in aversive learning .
	manualset3
179031	1	413845	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results for the first time suggest the possible role of HDAC2 in development of HAND .
	manualset3
179032	2	413845	7	NULL	NULL	0	NULL	first time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	These results for the first time suggest the possible role of HDAC2 in development of HAND .
	manualset3
179033	3	413845	7	NULL	NULL	0	NULL	 role 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results for the first time suggest the possible role of HDAC2 in development of HAND .
	manualset3
179034	4	413845	7	NULL	NULL	0	NULL	HDAC2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results for the first time suggest the possible role of HDAC2 in development of HAND .
	manualset3
179035	5	413845	7	NULL	NULL	NULL	NULL	development	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results for the first time suggest the possible role of HDAC2 in development of HAND .
	manualset3
179036	6	413845	7	NULL	NULL	0	NULL	HAND	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results for the first time suggest the possible role of HDAC2 in development of HAND .
	manualset3
179037	1	413846	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have demonstrated that a low load exercise protocol targeting the gluteal muscle group is effective at acutely enhancing peak power output in elite athletes .
	manualset3
179038	2	413846	7	NULL	NULL	0	NULL	 low load exercise protocol	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have demonstrated that a low load exercise protocol targeting the gluteal muscle group is effective at acutely enhancing peak power output in elite athletes .
	manualset3
179039	3	413846	7	NULL	NULL	0	NULL	gluteal muscle group	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have demonstrated that a low load exercise protocol targeting the gluteal muscle group is effective at acutely enhancing peak power output in elite athletes .
	manualset3
179040	4	413846	7	NULL	NULL	0	NULL	peak power output	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have demonstrated that a low load exercise protocol targeting the gluteal muscle group is effective at acutely enhancing peak power output in elite athletes .
	manualset3
179041	5	413846	7	NULL	NULL	0	NULL	elite athletes	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have demonstrated that a low load exercise protocol targeting the gluteal muscle group is effective at acutely enhancing peak power output in elite athletes .
	manualset3
179042	1	413847	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have demonstrated that there are diverse populations of cardiac ganglion cells in the guinea-pig and that some of these neurons may act as interneurons within the intrinsic cardiac plexuses .
	manualset3
179043	2	413847	7	NULL	NULL	0	NULL	 populations	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have demonstrated that there are diverse populations of cardiac ganglion cells in the guinea-pig and that some of these neurons may act as interneurons within the intrinsic cardiac plexuses .
	manualset3
179044	3	413847	7	NULL	NULL	0	NULL	cardiac ganglion cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have demonstrated that there are diverse populations of cardiac ganglion cells in the guinea-pig and that some of these neurons may act as interneurons within the intrinsic cardiac plexuses .
	manualset3
179045	4	413847	7	NULL	NULL	0	NULL	guinea-pig	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have demonstrated that there are diverse populations of cardiac ganglion cells in the guinea-pig and that some of these neurons may act as interneurons within the intrinsic cardiac plexuses .
	manualset3
179046	5	413847	7	NULL	NULL	0	NULL	neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have demonstrated that there are diverse populations of cardiac ganglion cells in the guinea-pig and that some of these neurons may act as interneurons within the intrinsic cardiac plexuses .
	manualset3
179047	6	413847	7	NULL	NULL	0	NULL	 interneurons 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have demonstrated that there are diverse populations of cardiac ganglion cells in the guinea-pig and that some of these neurons may act as interneurons within the intrinsic cardiac plexuses .
	manualset3
179048	7	413847	7	NULL	NULL	0	NULL	 intrinsic cardiac plexuses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have demonstrated that there are diverse populations of cardiac ganglion cells in the guinea-pig and that some of these neurons may act as interneurons within the intrinsic cardiac plexuses .
	manualset3
179049	1	413848	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have general implications for understanding the regulation of glycolysis , starch synthesis and other biosynthetic pathways in plants , and reveal a potential role for pyrophosphate in conserving energy and decreasing oxygen consumption .
	manualset3
179050	2	413848	7	NULL	NULL	0	NULL	implications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have general implications for understanding the regulation of glycolysis , starch synthesis and other biosynthetic pathways in plants , and reveal a potential role for pyrophosphate in conserving energy and decreasing oxygen consumption .
	manualset3
179051	3	413848	7	NULL	NULL	0	NULL	 regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have general implications for understanding the regulation of glycolysis , starch synthesis and other biosynthetic pathways in plants , and reveal a potential role for pyrophosphate in conserving energy and decreasing oxygen consumption .
	manualset3
179052	4	413848	7	NULL	NULL	0	NULL	glycolysis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have general implications for understanding the regulation of glycolysis , starch synthesis and other biosynthetic pathways in plants , and reveal a potential role for pyrophosphate in conserving energy and decreasing oxygen consumption .
	manualset3
179053	5	413848	7	NULL	NULL	0	NULL	 starch synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have general implications for understanding the regulation of glycolysis , starch synthesis and other biosynthetic pathways in plants , and reveal a potential role for pyrophosphate in conserving energy and decreasing oxygen consumption .
	manualset3
179054	6	413848	7	NULL	NULL	0	NULL	biosynthetic pathways	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have general implications for understanding the regulation of glycolysis , starch synthesis and other biosynthetic pathways in plants , and reveal a potential role for pyrophosphate in conserving energy and decreasing oxygen consumption .
	manualset3
179055	7	413848	7	NULL	NULL	0	NULL	plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have general implications for understanding the regulation of glycolysis , starch synthesis and other biosynthetic pathways in plants , and reveal a potential role for pyrophosphate in conserving energy and decreasing oxygen consumption .
	manualset3
179056	8	413848	7	NULL	NULL	0	NULL	 role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have general implications for understanding the regulation of glycolysis , starch synthesis and other biosynthetic pathways in plants , and reveal a potential role for pyrophosphate in conserving energy and decreasing oxygen consumption .
	manualset3
179057	9	413848	7	NULL	NULL	0	NULL	pyrophosphate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have general implications for understanding the regulation of glycolysis , starch synthesis and other biosynthetic pathways in plants , and reveal a potential role for pyrophosphate in conserving energy and decreasing oxygen consumption .
	manualset3
179058	10	413848	7	NULL	NULL	0	NULL	energy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have general implications for understanding the regulation of glycolysis , starch synthesis and other biosynthetic pathways in plants , and reveal a potential role for pyrophosphate in conserving energy and decreasing oxygen consumption .
	manualset3
179059	11	413848	7	NULL	NULL	0	NULL	oxygen consumption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have general implications for understanding the regulation of glycolysis , starch synthesis and other biosynthetic pathways in plants , and reveal a potential role for pyrophosphate in conserving energy and decreasing oxygen consumption .
	manualset3
179060	1	413849	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have implications for the genetic control of arcuate development and function and for the utility of the Nkx2.1-Cre and Dlx5/6i-Cre mouse lines to alter gene expression in the developing arcuate .
	manualset3
179061	2	413849	7	NULL	NULL	0	NULL	implications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have implications for the genetic control of arcuate development and function and for the utility of the Nkx2.1-Cre and Dlx5/6i-Cre mouse lines to alter gene expression in the developing arcuate .
	manualset3
179062	3	413849	7	NULL	NULL	0	NULL	genetic control 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have implications for the genetic control of arcuate development and function and for the utility of the Nkx2.1-Cre and Dlx5/6i-Cre mouse lines to alter gene expression in the developing arcuate .
	manualset3
179064	4	413849	7	NULL	NULL	0	NULL	arcuate development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have implications for the genetic control of arcuate development and function and for the utility of the Nkx2.1-Cre and Dlx5/6i-Cre mouse lines to alter gene expression in the developing arcuate .
	manualset3
179065	5	413849	7	NULL	NULL	0	NULL	function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have implications for the genetic control of arcuate development and function and for the utility of the Nkx2.1-Cre and Dlx5/6i-Cre mouse lines to alter gene expression in the developing arcuate .
	manualset3
179066	6	413849	7	NULL	NULL	0	NULL	utility	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have implications for the genetic control of arcuate development and function and for the utility of the Nkx2.1-Cre and Dlx5/6i-Cre mouse lines to alter gene expression in the developing arcuate .
	manualset3
179067	7	413849	7	NULL	NULL	0	NULL	Nkx2.1-Cre mouse lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have implications for the genetic control of arcuate development and function and for the utility of the Nkx2.1-Cre and Dlx5/6i-Cre mouse lines to alter gene expression in the developing arcuate .
	manualset3
179068	8	413849	7	NULL	NULL	0	NULL	Dlx5/6i-Cre mouse lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have implications for the genetic control of arcuate development and function and for the utility of the Nkx2.1-Cre and Dlx5/6i-Cre mouse lines to alter gene expression in the developing arcuate .
	manualset3
179069	9	413849	7	NULL	NULL	0	NULL	gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have implications for the genetic control of arcuate development and function and for the utility of the Nkx2.1-Cre and Dlx5/6i-Cre mouse lines to alter gene expression in the developing arcuate .
	manualset3
179070	10	413849	7	NULL	NULL	0	NULL	developing arcuate	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results have implications for the genetic control of arcuate development and function and for the utility of the Nkx2.1-Cre and Dlx5/6i-Cre mouse lines to alter gene expression in the developing arcuate .
	manualset3
179071	1	413850	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results highlight important gender differences that exist in the current clinical definitions of the metabolic syndrome , with regards to predicting early atherosclerotic lesions .
	manualset3
179072	2	413850	7	NULL	NULL	0	NULL	gender differences	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results highlight important gender differences that exist in the current clinical definitions of the metabolic syndrome , with regards to predicting early atherosclerotic lesions .
	manualset3
179073	3	413850	7	NULL	NULL	0	NULL	clinical definitions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results highlight important gender differences that exist in the current clinical definitions of the metabolic syndrome , with regards to predicting early atherosclerotic lesions .
	manualset3
179074	4	413850	7	NULL	NULL	0	NULL	metabolic syndrome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results highlight important gender differences that exist in the current clinical definitions of the metabolic syndrome , with regards to predicting early atherosclerotic lesions .
	manualset3
179075	5	413850	7	NULL	NULL	0	NULL	early atherosclerotic lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results highlight important gender differences that exist in the current clinical definitions of the metabolic syndrome , with regards to predicting early atherosclerotic lesions .
	manualset3
179076	1	413851	7	NULL	NULL	0	NULL	Additional studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional studies are needed to examine the role of autoregulatory systems in the development of WMH , particularly those using beat-to-beat measures of BP .
	manualset3
179077	2	413851	7	NULL	NULL	0	NULL	 role 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional studies are needed to examine the role of autoregulatory systems in the development of WMH , particularly those using beat-to-beat measures of BP .
	manualset3
179078	3	413851	7	NULL	NULL	0	NULL	autoregulatory systems	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional studies are needed to examine the role of autoregulatory systems in the development of WMH , particularly those using beat-to-beat measures of BP .
	manualset3
179079	4	413851	7	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional studies are needed to examine the role of autoregulatory systems in the development of WMH , particularly those using beat-to-beat measures of BP .
	manualset3
179080	5	413851	7	NULL	NULL	0	NULL	WMH	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional studies are needed to examine the role of autoregulatory systems in the development of WMH , particularly those using beat-to-beat measures of BP .
	manualset3
179081	6	413851	7	NULL	NULL	0	NULL	beat-to-beat measures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional studies are needed to examine the role of autoregulatory systems in the development of WMH , particularly those using beat-to-beat measures of BP .
	manualset3
179082	7	413851	7	NULL	NULL	0	NULL	BP	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional studies are needed to examine the role of autoregulatory systems in the development of WMH , particularly those using beat-to-beat measures of BP .
	manualset3
179083	1	413852	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results identify Kir5 .1 as an important determinant of PCO ( 2 ) / pH sensitivity in locus coeruleus neurons and suggest that Kir5 .1 may be involved in the response to hypercapnic acidosis .
	manualset3
179084	2	413852	7	NULL	NULL	0	NULL	Kir5 .1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results identify Kir5 .1 as an important determinant of PCO ( 2 ) / pH sensitivity in locus coeruleus neurons and suggest that Kir5 .1 may be involved in the response to hypercapnic acidosis .
	manualset3
179085	3	413852	7	NULL	NULL	0	NULL	PCO ( 2 ) / pH sensitivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results identify Kir5 .1 as an important determinant of PCO ( 2 ) / pH sensitivity in locus coeruleus neurons and suggest that Kir5 .1 may be involved in the response to hypercapnic acidosis .
	manualset3
179086	4	413852	7	NULL	NULL	0	NULL	locus coeruleus neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results identify Kir5 .1 as an important determinant of PCO ( 2 ) / pH sensitivity in locus coeruleus neurons and suggest that Kir5 .1 may be involved in the response to hypercapnic acidosis .
	manualset3
179087	5	413852	7	NULL	NULL	0	NULL	 Kir5 .1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results identify Kir5 .1 as an important determinant of PCO ( 2 ) / pH sensitivity in locus coeruleus neurons and suggest that Kir5 .1 may be involved in the response to hypercapnic acidosis .
	manualset3
179088	6	413852	7	NULL	NULL	0	NULL	hypercapnic acidosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results identify Kir5 .1 as an important determinant of PCO ( 2 ) / pH sensitivity in locus coeruleus neurons and suggest that Kir5 .1 may be involved in the response to hypercapnic acidosis .
	manualset3
181842	7	413852	7	NULL	NULL	0	NULL	response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results identify Kir5 .1 as an important determinant of PCO ( 2 ) / pH sensitivity in locus coeruleus neurons and suggest that Kir5 .1 may be involved in the response to hypercapnic acidosis .
	manualset3
179089	1	413853	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results identify a novel mechanism of transcriptional enhancement involving ligand-independent activity of the VDR/RXR heterodimer and MAPK signaling pathways that appears to play an important role in the overexpression of PDGF in many different settings of human malignancy .
	manualset3
179090	2	413853	7	NULL	NULL	0	NULL	novel mechanism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results identify a novel mechanism of transcriptional enhancement involving ligand-independent activity of the VDR/RXR heterodimer and MAPK signaling pathways that appears to play an important role in the overexpression of PDGF in many different settings of human malignancy .
	manualset3
179091	3	413853	7	NULL	NULL	0	NULL	transcriptional enhancement	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results identify a novel mechanism of transcriptional enhancement involving ligand-independent activity of the VDR/RXR heterodimer and MAPK signaling pathways that appears to play an important role in the overexpression of PDGF in many different settings of human malignancy .
	manualset3
179092	4	413853	7	NULL	NULL	NULL	NULL	ligand-independent activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results identify a novel mechanism of transcriptional enhancement involving ligand-independent activity of the VDR/RXR heterodimer and MAPK signaling pathways that appears to play an important role in the overexpression of PDGF in many different settings of human malignancy .
	manualset3
179093	5	413853	7	NULL	NULL	0	NULL	VDR/RXR heterodimer	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results identify a novel mechanism of transcriptional enhancement involving ligand-independent activity of the VDR/RXR heterodimer and MAPK signaling pathways that appears to play an important role in the overexpression of PDGF in many different settings of human malignancy .
	manualset3
179094	6	413853	7	NULL	NULL	0	NULL	MAPK signaling pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results identify a novel mechanism of transcriptional enhancement involving ligand-independent activity of the VDR/RXR heterodimer and MAPK signaling pathways that appears to play an important role in the overexpression of PDGF in many different settings of human malignancy .
	manualset3
179095	7	413853	7	NULL	NULL	0	NULL	 role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results identify a novel mechanism of transcriptional enhancement involving ligand-independent activity of the VDR/RXR heterodimer and MAPK signaling pathways that appears to play an important role in the overexpression of PDGF in many different settings of human malignancy .
	manualset3
179096	8	413853	7	NULL	NULL	0	NULL	overexpression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results identify a novel mechanism of transcriptional enhancement involving ligand-independent activity of the VDR/RXR heterodimer and MAPK signaling pathways that appears to play an important role in the overexpression of PDGF in many different settings of human malignancy .
	manualset3
179097	9	413853	7	NULL	NULL	0	NULL	PDGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results identify a novel mechanism of transcriptional enhancement involving ligand-independent activity of the VDR/RXR heterodimer and MAPK signaling pathways that appears to play an important role in the overexpression of PDGF in many different settings of human malignancy .
	manualset3
179098	10	413853	7	NULL	NULL	0	NULL	human malignancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results identify a novel mechanism of transcriptional enhancement involving ligand-independent activity of the VDR/RXR heterodimer and MAPK signaling pathways that appears to play an important role in the overexpression of PDGF in many different settings of human malignancy .
	manualset3
179099	1	413854	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results illustrate aspects of assay performance which may be overlooked once a formal `` validation exercise '' has been carried out and assays are in routine use .
	manualset3
179100	2	413854	7	NULL	NULL	0	NULL	assay performance	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results illustrate aspects of assay performance which may be overlooked once a formal `` validation exercise '' has been carried out and assays are in routine use .
	manualset3
179101	3	413854	7	NULL	NULL	0	NULL	validation exercise	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These results illustrate aspects of assay performance which may be overlooked once a formal `` validation exercise '' has been carried out and assays are in routine use .
	manualset3
179102	4	413854	7	NULL	NULL	0	NULL	assays 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results illustrate aspects of assay performance which may be overlooked once a formal `` validation exercise '' has been carried out and assays are in routine use .
	manualset3
179103	1	413855	7	NULL	NULL	0	NULL	 results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results implicate CaMKII as a molecular messenger in the acquisition of PTZ kindling .
	manualset3
179104	2	413855	7	NULL	NULL	0	NULL	CaMKII	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results implicate CaMKII as a molecular messenger in the acquisition of PTZ kindling .
	manualset3
179105	3	413855	7	NULL	NULL	0	NULL	 molecular messenger	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results implicate CaMKII as a molecular messenger in the acquisition of PTZ kindling .
	manualset3
179106	4	413855	7	NULL	NULL	0	NULL	acquisition 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results implicate CaMKII as a molecular messenger in the acquisition of PTZ kindling .
	manualset3
179107	5	413855	7	NULL	NULL	0	NULL	PTZ kindling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results implicate CaMKII as a molecular messenger in the acquisition of PTZ kindling .
	manualset3
179108	1	413856	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results implied that 18F-AMT was metabolized to protein to only a small extent and trapped as intact 18F-AMT in cells up to 60 min .
	manualset3
179109	2	413856	7	NULL	NULL	0	NULL	18F-AMT	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results implied that 18F-AMT was metabolized to protein to only a small extent and trapped as intact 18F-AMT in cells up to 60 min .
	manualset3
179110	3	413856	7	NULL	NULL	0	NULL	protein	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results implied that 18F-AMT was metabolized to protein to only a small extent and trapped as intact 18F-AMT in cells up to 60 min .
	manualset3
179111	4	413856	7	NULL	NULL	0	NULL	small extent	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results implied that 18F-AMT was metabolized to protein to only a small extent and trapped as intact 18F-AMT in cells up to 60 min .
	manualset3
179112	5	413856	7	NULL	NULL	0	NULL	 18F-AMT	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results implied that 18F-AMT was metabolized to protein to only a small extent and trapped as intact 18F-AMT in cells up to 60 min .
	manualset3
179113	6	413856	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results implied that 18F-AMT was metabolized to protein to only a small extent and trapped as intact 18F-AMT in cells up to 60 min .
	manualset3
179114	7	413856	7	NULL	NULL	0	NULL	60 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	These results implied that 18F-AMT was metabolized to protein to only a small extent and trapped as intact 18F-AMT in cells up to 60 min .
	manualset3
179115	1	413857	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results imply that changes in P ' L especially affect Phr activity early in inspiration .
	manualset3
179116	2	413857	7	NULL	NULL	0	NULL	changes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results imply that changes in P ' L especially affect Phr activity early in inspiration .
	manualset3
179117	3	413857	7	NULL	NULL	0	NULL	P ' L	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results imply that changes in P ' L especially affect Phr activity early in inspiration .
	manualset3
179118	4	413857	7	NULL	NULL	0	NULL	Phr activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results imply that changes in P ' L especially affect Phr activity early in inspiration .
	manualset3
179119	5	413857	7	NULL	NULL	0	NULL	inspiration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results imply that changes in P ' L especially affect Phr activity early in inspiration .
	manualset3
179120	1	413858	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate a model whereby Pou3f4 in the otic mesenchyme establishes an Eph/ephrin-mediated fasciculation signal that promotes inner radial bundle formation .
	manualset3
179121	2	413858	7	NULL	NULL	NULL	NULL	model	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results indicate a model whereby Pou3f4 in the otic mesenchyme establishes an Eph/ephrin-mediated fasciculation signal that promotes inner radial bundle formation .
	manualset3
179122	3	413858	7	NULL	NULL	0	NULL	Pou3f4 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate a model whereby Pou3f4 in the otic mesenchyme establishes an Eph/ephrin-mediated fasciculation signal that promotes inner radial bundle formation .
	manualset3
179123	4	413858	7	NULL	NULL	0	NULL	otic mesenchyme	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate a model whereby Pou3f4 in the otic mesenchyme establishes an Eph/ephrin-mediated fasciculation signal that promotes inner radial bundle formation .
	manualset3
179124	5	413858	7	NULL	NULL	0	NULL	Eph/ephrin-mediated fasciculation signal 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate a model whereby Pou3f4 in the otic mesenchyme establishes an Eph/ephrin-mediated fasciculation signal that promotes inner radial bundle formation .
	manualset3
179125	6	413858	7	NULL	NULL	0	NULL	inner radial bundle formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate a model whereby Pou3f4 in the otic mesenchyme establishes an Eph/ephrin-mediated fasciculation signal that promotes inner radial bundle formation .
	manualset3
179126	1	413859	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate a need for a multi-ethnic approach to the assessment and treatment of sleep disorders .
	manualset3
179127	2	413859	7	NULL	NULL	0	NULL	multi-ethnic approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate a need for a multi-ethnic approach to the assessment and treatment of sleep disorders .
	manualset3
179128	3	413859	7	NULL	NULL	0	NULL	assessment 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate a need for a multi-ethnic approach to the assessment and treatment of sleep disorders .
	manualset3
179129	4	413859	7	NULL	NULL	0	NULL	treatment 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate a need for a multi-ethnic approach to the assessment and treatment of sleep disorders .
	manualset3
179130	5	413859	7	NULL	NULL	0	NULL	sleep disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate a need for a multi-ethnic approach to the assessment and treatment of sleep disorders .
	manualset3
179131	1	413860	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate a role for thrombospondin as an important mediator of staphylococcal adherence to activated platelets , to blood clots , or to extracellular matrices in pyogenic infections .
	manualset3
179132	2	413860	7	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate a role for thrombospondin as an important mediator of staphylococcal adherence to activated platelets , to blood clots , or to extracellular matrices in pyogenic infections .
	manualset3
179133	3	413860	7	NULL	NULL	0	NULL	thrombospondin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate a role for thrombospondin as an important mediator of staphylococcal adherence to activated platelets , to blood clots , or to extracellular matrices in pyogenic infections .
	manualset3
179134	4	413860	7	NULL	NULL	0	NULL	mediator	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate a role for thrombospondin as an important mediator of staphylococcal adherence to activated platelets , to blood clots , or to extracellular matrices in pyogenic infections .
	manualset3
179135	5	413860	7	NULL	NULL	0	NULL	staphylococcal adherence 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate a role for thrombospondin as an important mediator of staphylococcal adherence to activated platelets , to blood clots , or to extracellular matrices in pyogenic infections .
	manualset3
179136	6	413860	7	NULL	NULL	0	NULL	activated platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate a role for thrombospondin as an important mediator of staphylococcal adherence to activated platelets , to blood clots , or to extracellular matrices in pyogenic infections .
	manualset3
179137	7	413860	7	NULL	NULL	0	NULL	blood clots	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate a role for thrombospondin as an important mediator of staphylococcal adherence to activated platelets , to blood clots , or to extracellular matrices in pyogenic infections .
	manualset3
179138	8	413860	7	NULL	NULL	0	NULL	extracellular matrices	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate a role for thrombospondin as an important mediator of staphylococcal adherence to activated platelets , to blood clots , or to extracellular matrices in pyogenic infections .
	manualset3
179139	9	413860	7	NULL	NULL	0	NULL	pyogenic infections 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate a role for thrombospondin as an important mediator of staphylococcal adherence to activated platelets , to blood clots , or to extracellular matrices in pyogenic infections .
	manualset3
179140	1	413861	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate an essential pro-proliferative and pro-survival role for PKCalpha in glioma but question the use of ATP competitive inhibitors as therapeutics , either alone , or in combination with chemotoxic agents .
	manualset3
179141	2	413861	7	NULL	NULL	0	NULL	 essential pro-proliferative role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate an essential pro-proliferative and pro-survival role for PKCalpha in glioma but question the use of ATP competitive inhibitors as therapeutics , either alone , or in combination with chemotoxic agents .
	manualset3
179142	3	413861	7	NULL	NULL	0	NULL	pro-survival role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate an essential pro-proliferative and pro-survival role for PKCalpha in glioma but question the use of ATP competitive inhibitors as therapeutics , either alone , or in combination with chemotoxic agents .
	manualset3
179143	4	413861	7	NULL	NULL	0	NULL	PKCalpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate an essential pro-proliferative and pro-survival role for PKCalpha in glioma but question the use of ATP competitive inhibitors as therapeutics , either alone , or in combination with chemotoxic agents .
	manualset3
179144	5	413861	7	NULL	NULL	0	NULL	glioma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate an essential pro-proliferative and pro-survival role for PKCalpha in glioma but question the use of ATP competitive inhibitors as therapeutics , either alone , or in combination with chemotoxic agents .
	manualset3
179145	6	413861	7	NULL	NULL	0	NULL	ATP competitive inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate an essential pro-proliferative and pro-survival role for PKCalpha in glioma but question the use of ATP competitive inhibitors as therapeutics , either alone , or in combination with chemotoxic agents .
	manualset3
179146	7	413861	7	NULL	NULL	0	NULL	therapeutics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate an essential pro-proliferative and pro-survival role for PKCalpha in glioma but question the use of ATP competitive inhibitors as therapeutics , either alone , or in combination with chemotoxic agents .
	manualset3
179147	8	413861	7	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate an essential pro-proliferative and pro-survival role for PKCalpha in glioma but question the use of ATP competitive inhibitors as therapeutics , either alone , or in combination with chemotoxic agents .
	manualset3
179148	9	413861	7	NULL	NULL	0	NULL	chemotoxic agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate an essential pro-proliferative and pro-survival role for PKCalpha in glioma but question the use of ATP competitive inhibitors as therapeutics , either alone , or in combination with chemotoxic agents .
	manualset3
179170	1	413862	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional studies indicated that a putative promoting agent , such as phenobarbital , increased the incidence of those tumor types usually associated with spontaneous appearance and only in strains with a genetic predisposition to spontaneous tumorigenesis .
	manualset3
179171	2	413862	7	NULL	NULL	0	NULL	putative promoting agent	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional studies indicated that a putative promoting agent , such as phenobarbital , increased the incidence of those tumor types usually associated with spontaneous appearance and only in strains with a genetic predisposition to spontaneous tumorigenesis .
	manualset3
179172	3	413862	7	NULL	NULL	0	NULL	phenobarbital	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional studies indicated that a putative promoting agent , such as phenobarbital , increased the incidence of those tumor types usually associated with spontaneous appearance and only in strains with a genetic predisposition to spontaneous tumorigenesis .
	manualset3
179173	4	413862	7	NULL	NULL	0	NULL	incidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional studies indicated that a putative promoting agent , such as phenobarbital , increased the incidence of those tumor types usually associated with spontaneous appearance and only in strains with a genetic predisposition to spontaneous tumorigenesis .
	manualset3
179174	5	413862	7	NULL	NULL	0	NULL	tumor types	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional studies indicated that a putative promoting agent , such as phenobarbital , increased the incidence of those tumor types usually associated with spontaneous appearance and only in strains with a genetic predisposition to spontaneous tumorigenesis .
	manualset3
179175	6	413862	7	NULL	NULL	0	NULL	strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional studies indicated that a putative promoting agent , such as phenobarbital , increased the incidence of those tumor types usually associated with spontaneous appearance and only in strains with a genetic predisposition to spontaneous tumorigenesis .
	manualset3
179177	7	413862	7	NULL	NULL	0	NULL	genetic predisposition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional studies indicated that a putative promoting agent , such as phenobarbital , increased the incidence of those tumor types usually associated with spontaneous appearance and only in strains with a genetic predisposition to spontaneous tumorigenesis .
	manualset3
179178	8	413862	7	NULL	NULL	0	NULL	spontaneous tumorigenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional studies indicated that a putative promoting agent , such as phenobarbital , increased the incidence of those tumor types usually associated with spontaneous appearance and only in strains with a genetic predisposition to spontaneous tumorigenesis .
	manualset3
182012	9	413862	7	NULL	NULL	0	NULL	spontaneous appearance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional studies indicated that a putative promoting agent , such as phenobarbital , increased the incidence of those tumor types usually associated with spontaneous appearance and only in strains with a genetic predisposition to spontaneous tumorigenesis .
	manualset3
179250	1	413863	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that , despite considerable plasma volume expansion , HA infusion does not enhance Na excretion in Na-restricted subjects .
	manualset3
179251	2	413863	7	NULL	NULL	0	NULL	plasma volume expansion	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that , despite considerable plasma volume expansion , HA infusion does not enhance Na excretion in Na-restricted subjects .
	manualset3
179252	3	413863	7	NULL	NULL	0	NULL	HA infusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that , despite considerable plasma volume expansion , HA infusion does not enhance Na excretion in Na-restricted subjects .
	manualset3
179253	4	413863	7	NULL	NULL	0	NULL	Na excretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that , despite considerable plasma volume expansion , HA infusion does not enhance Na excretion in Na-restricted subjects .
	manualset3
179254	5	413863	7	NULL	NULL	0	NULL	Na-restricted subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that , despite considerable plasma volume expansion , HA infusion does not enhance Na excretion in Na-restricted subjects .
	manualset3
179255	1	413864	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that , in Dahl rats , the postabsorptive mechanism plays a significant role in controlling long-term saline drinking behavior and Na + balance and has a significant role in controlling arterial pressure in DS , but not DR , rats .
	manualset3
179256	2	413864	7	NULL	NULL	0	NULL	Dahl rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that , in Dahl rats , the postabsorptive mechanism plays a significant role in controlling long-term saline drinking behavior and Na + balance and has a significant role in controlling arterial pressure in DS , but not DR , rats .
	manualset3
179258	3	413864	7	NULL	NULL	0	NULL	postabsorptive mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that , in Dahl rats , the postabsorptive mechanism plays a significant role in controlling long-term saline drinking behavior and Na + balance and has a significant role in controlling arterial pressure in DS , but not DR , rats .
	manualset3
179261	4	413864	7	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that , in Dahl rats , the postabsorptive mechanism plays a significant role in controlling long-term saline drinking behavior and Na + balance and has a significant role in controlling arterial pressure in DS , but not DR , rats .
	manualset3
179262	5	413864	7	NULL	NULL	NULL	NULL	long-term saline drinking behavior	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results indicate that , in Dahl rats , the postabsorptive mechanism plays a significant role in controlling long-term saline drinking behavior and Na + balance and has a significant role in controlling arterial pressure in DS , but not DR , rats .
	manualset3
179263	6	413864	7	NULL	NULL	0	NULL	Na + balance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that , in Dahl rats , the postabsorptive mechanism plays a significant role in controlling long-term saline drinking behavior and Na + balance and has a significant role in controlling arterial pressure in DS , but not DR , rats .
	manualset3
179264	7	413864	7	NULL	NULL	0	NULL	 role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that , in Dahl rats , the postabsorptive mechanism plays a significant role in controlling long-term saline drinking behavior and Na + balance and has a significant role in controlling arterial pressure in DS , but not DR , rats .
	manualset3
179265	8	413864	7	NULL	NULL	0	NULL	arterial pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that , in Dahl rats , the postabsorptive mechanism plays a significant role in controlling long-term saline drinking behavior and Na + balance and has a significant role in controlling arterial pressure in DS , but not DR , rats .
	manualset3
179266	9	413864	7	NULL	NULL	0	NULL	DS rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that , in Dahl rats , the postabsorptive mechanism plays a significant role in controlling long-term saline drinking behavior and Na + balance and has a significant role in controlling arterial pressure in DS , but not DR , rats .
	manualset3
179268	10	413864	7	NULL	NULL	0	NULL	DR  rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that , in Dahl rats , the postabsorptive mechanism plays a significant role in controlling long-term saline drinking behavior and Na + balance and has a significant role in controlling arterial pressure in DS , but not DR , rats .
	manualset3
182013	11	413864	7	NULL	NULL	0	NULL	controlling	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that , in Dahl rats , the postabsorptive mechanism plays a significant role in controlling long-term saline drinking behavior and Na + balance and has a significant role in controlling arterial pressure in DS , but not DR , rats .
	manualset3
179277	1	413865	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that Ag ( I ) induced in the DNA-alginate film keeps the potent antibacterial activity , and so DNA is very useful as a carrier of silver ion in the alginate film .
	manualset3
179279	2	413865	7	NULL	NULL	0	NULL	Ag ( I )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that Ag ( I ) induced in the DNA-alginate film keeps the potent antibacterial activity , and so DNA is very useful as a carrier of silver ion in the alginate film .
	manualset3
179283	3	413865	7	NULL	NULL	0	NULL	DNA-alginate film 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that Ag ( I ) induced in the DNA-alginate film keeps the potent antibacterial activity , and so DNA is very useful as a carrier of silver ion in the alginate film .
	manualset3
179284	4	413865	7	NULL	NULL	0	NULL	antibacterial activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that Ag ( I ) induced in the DNA-alginate film keeps the potent antibacterial activity , and so DNA is very useful as a carrier of silver ion in the alginate film .
	manualset3
179285	5	413865	7	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that Ag ( I ) induced in the DNA-alginate film keeps the potent antibacterial activity , and so DNA is very useful as a carrier of silver ion in the alginate film .
	manualset3
179291	6	413865	7	NULL	NULL	NULL	NULL	carrier	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results indicate that Ag ( I ) induced in the DNA-alginate film keeps the potent antibacterial activity , and so DNA is very useful as a carrier of silver ion in the alginate film .
	manualset3
179293	7	413865	7	NULL	NULL	0	NULL	silver ion	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that Ag ( I ) induced in the DNA-alginate film keeps the potent antibacterial activity , and so DNA is very useful as a carrier of silver ion in the alginate film .
	manualset3
179294	8	413865	7	NULL	NULL	0	NULL	alginate film	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that Ag ( I ) induced in the DNA-alginate film keeps the potent antibacterial activity , and so DNA is very useful as a carrier of silver ion in the alginate film .
	manualset3
179298	1	413866	7	NULL	NULL	0	NULL	 results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that CRA inhibits gluconeogenesis by increasing the production of F-2 , 6 - BP by lowering the cAMP level and inhibiting PKA activity in isolated hepatocytes .
	manualset3
179299	2	413866	7	NULL	NULL	0	NULL	CRA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that CRA inhibits gluconeogenesis by increasing the production of F-2 , 6 - BP by lowering the cAMP level and inhibiting PKA activity in isolated hepatocytes .
	manualset3
179300	3	413866	7	NULL	NULL	NULL	NULL	gluconeogenesis 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results indicate that CRA inhibits gluconeogenesis by increasing the production of F-2 , 6 - BP by lowering the cAMP level and inhibiting PKA activity in isolated hepatocytes .
	manualset3
179301	4	413866	7	NULL	NULL	0	NULL	production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that CRA inhibits gluconeogenesis by increasing the production of F-2 , 6 - BP by lowering the cAMP level and inhibiting PKA activity in isolated hepatocytes .
	manualset3
179302	5	413866	7	NULL	NULL	0	NULL	F-2 , 6 - BP	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that CRA inhibits gluconeogenesis by increasing the production of F-2 , 6 - BP by lowering the cAMP level and inhibiting PKA activity in isolated hepatocytes .
	manualset3
179303	6	413866	7	NULL	NULL	0	NULL	cAMP level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that CRA inhibits gluconeogenesis by increasing the production of F-2 , 6 - BP by lowering the cAMP level and inhibiting PKA activity in isolated hepatocytes .
	manualset3
179304	7	413866	7	NULL	NULL	NULL	NULL	PKA activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results indicate that CRA inhibits gluconeogenesis by increasing the production of F-2 , 6 - BP by lowering the cAMP level and inhibiting PKA activity in isolated hepatocytes .
	manualset3
179305	8	413866	7	NULL	NULL	0	NULL	isolated hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that CRA inhibits gluconeogenesis by increasing the production of F-2 , 6 - BP by lowering the cAMP level and inhibiting PKA activity in isolated hepatocytes .
	manualset3
182014	9	413866	7	NULL	NULL	0	NULL	lowering	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that CRA inhibits gluconeogenesis by increasing the production of F-2 , 6 - BP by lowering the cAMP level and inhibiting PKA activity in isolated hepatocytes .
	manualset3
182015	10	413866	7	NULL	NULL	0	NULL	 inhibiting	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that CRA inhibits gluconeogenesis by increasing the production of F-2 , 6 - BP by lowering the cAMP level and inhibiting PKA activity in isolated hepatocytes .
	manualset3
179306	1	413867	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that DAPK does not regulate radiation-induced cell death and that it can not be either a target molecule for radiotherapy with gene therapy or a prognostic marker for cervical cancer patients treated with radiotherapy .
	manualset3
179307	2	413867	7	NULL	NULL	0	NULL	DAPK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that DAPK does not regulate radiation-induced cell death and that it can not be either a target molecule for radiotherapy with gene therapy or a prognostic marker for cervical cancer patients treated with radiotherapy .
	manualset3
179308	3	413867	7	NULL	NULL	0	NULL	radiation-induced cell death 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that DAPK does not regulate radiation-induced cell death and that it can not be either a target molecule for radiotherapy with gene therapy or a prognostic marker for cervical cancer patients treated with radiotherapy .
	manualset3
179309	4	413867	7	NULL	NULL	0	NULL	target molecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that DAPK does not regulate radiation-induced cell death and that it can not be either a target molecule for radiotherapy with gene therapy or a prognostic marker for cervical cancer patients treated with radiotherapy .
	manualset3
179310	5	413867	7	NULL	NULL	0	NULL	radiotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that DAPK does not regulate radiation-induced cell death and that it can not be either a target molecule for radiotherapy with gene therapy or a prognostic marker for cervical cancer patients treated with radiotherapy .
	manualset3
179311	6	413867	7	NULL	NULL	0	NULL	gene therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that DAPK does not regulate radiation-induced cell death and that it can not be either a target molecule for radiotherapy with gene therapy or a prognostic marker for cervical cancer patients treated with radiotherapy .
	manualset3
179312	7	413867	7	NULL	NULL	0	NULL	prognostic marker	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that DAPK does not regulate radiation-induced cell death and that it can not be either a target molecule for radiotherapy with gene therapy or a prognostic marker for cervical cancer patients treated with radiotherapy .
	manualset3
179313	8	413867	7	NULL	NULL	0	NULL	cervical cancer patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that DAPK does not regulate radiation-induced cell death and that it can not be either a target molecule for radiotherapy with gene therapy or a prognostic marker for cervical cancer patients treated with radiotherapy .
	manualset3
179314	9	413867	7	NULL	NULL	0	NULL	radiotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that DAPK does not regulate radiation-induced cell death and that it can not be either a target molecule for radiotherapy with gene therapy or a prognostic marker for cervical cancer patients treated with radiotherapy .
	manualset3
179315	1	413868	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that HCV-core functions as a positive regulator of IGF-II transcription through the PKC pathway and that Sp1 and Egr1 are direct targets of the transcriptional regulation of the IGF-II gene which plays an important role in hepatitis C virus pathogenesis during the formation of hepatocellular carcinoma ( HCC ) .
	manualset3
179316	2	413868	7	NULL	NULL	0	NULL	HCV-core	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that HCV-core functions as a positive regulator of IGF-II transcription through the PKC pathway and that Sp1 and Egr1 are direct targets of the transcriptional regulation of the IGF-II gene which plays an important role in hepatitis C virus pathogenesis during the formation of hepatocellular carcinoma ( HCC ) .
	manualset3
179317	3	413868	7	NULL	NULL	0	NULL	positive regulator	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that HCV-core functions as a positive regulator of IGF-II transcription through the PKC pathway and that Sp1 and Egr1 are direct targets of the transcriptional regulation of the IGF-II gene which plays an important role in hepatitis C virus pathogenesis during the formation of hepatocellular carcinoma ( HCC ) .
	manualset3
179318	4	413868	7	NULL	NULL	0	NULL	IGF-II transcription 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that HCV-core functions as a positive regulator of IGF-II transcription through the PKC pathway and that Sp1 and Egr1 are direct targets of the transcriptional regulation of the IGF-II gene which plays an important role in hepatitis C virus pathogenesis during the formation of hepatocellular carcinoma ( HCC ) .
	manualset3
179319	5	413868	7	NULL	NULL	0	NULL	PKC pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that HCV-core functions as a positive regulator of IGF-II transcription through the PKC pathway and that Sp1 and Egr1 are direct targets of the transcriptional regulation of the IGF-II gene which plays an important role in hepatitis C virus pathogenesis during the formation of hepatocellular carcinoma ( HCC ) .
	manualset3
179320	6	413868	7	NULL	NULL	0	NULL	 Sp1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that HCV-core functions as a positive regulator of IGF-II transcription through the PKC pathway and that Sp1 and Egr1 are direct targets of the transcriptional regulation of the IGF-II gene which plays an important role in hepatitis C virus pathogenesis during the formation of hepatocellular carcinoma ( HCC ) .
	manualset3
179321	7	413868	7	NULL	NULL	0	NULL	Egr1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that HCV-core functions as a positive regulator of IGF-II transcription through the PKC pathway and that Sp1 and Egr1 are direct targets of the transcriptional regulation of the IGF-II gene which plays an important role in hepatitis C virus pathogenesis during the formation of hepatocellular carcinoma ( HCC ) .
	manualset3
179322	8	413868	7	NULL	NULL	0	NULL	targets 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that HCV-core functions as a positive regulator of IGF-II transcription through the PKC pathway and that Sp1 and Egr1 are direct targets of the transcriptional regulation of the IGF-II gene which plays an important role in hepatitis C virus pathogenesis during the formation of hepatocellular carcinoma ( HCC ) .
	manualset3
179323	9	413868	7	NULL	NULL	0	NULL	transcriptional regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that HCV-core functions as a positive regulator of IGF-II transcription through the PKC pathway and that Sp1 and Egr1 are direct targets of the transcriptional regulation of the IGF-II gene which plays an important role in hepatitis C virus pathogenesis during the formation of hepatocellular carcinoma ( HCC ) .
	manualset3
179324	10	413868	7	NULL	NULL	0	NULL	IGF-II gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that HCV-core functions as a positive regulator of IGF-II transcription through the PKC pathway and that Sp1 and Egr1 are direct targets of the transcriptional regulation of the IGF-II gene which plays an important role in hepatitis C virus pathogenesis during the formation of hepatocellular carcinoma ( HCC ) .
	manualset3
179325	11	413868	7	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that HCV-core functions as a positive regulator of IGF-II transcription through the PKC pathway and that Sp1 and Egr1 are direct targets of the transcriptional regulation of the IGF-II gene which plays an important role in hepatitis C virus pathogenesis during the formation of hepatocellular carcinoma ( HCC ) .
	manualset3
179326	12	413868	7	NULL	NULL	NULL	NULL	hepatitis C virus pathogenesis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results indicate that HCV-core functions as a positive regulator of IGF-II transcription through the PKC pathway and that Sp1 and Egr1 are direct targets of the transcriptional regulation of the IGF-II gene which plays an important role in hepatitis C virus pathogenesis during the formation of hepatocellular carcinoma ( HCC ) .
	manualset3
179327	13	413868	7	NULL	NULL	NULL	NULL	formation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results indicate that HCV-core functions as a positive regulator of IGF-II transcription through the PKC pathway and that Sp1 and Egr1 are direct targets of the transcriptional regulation of the IGF-II gene which plays an important role in hepatitis C virus pathogenesis during the formation of hepatocellular carcinoma ( HCC ) .
	manualset3
179328	14	413868	7	NULL	NULL	0	NULL	hepatocellular carcinoma ( HCC )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that HCV-core functions as a positive regulator of IGF-II transcription through the PKC pathway and that Sp1 and Egr1 are direct targets of the transcriptional regulation of the IGF-II gene which plays an important role in hepatitis C virus pathogenesis during the formation of hepatocellular carcinoma ( HCC ) .
	manualset3
179329	1	413869	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that N-cadherin may be a critical cell-to-cell adhesion molecule between corneal epithelial stem/progenitor cells and their corresponding niche cells in the limbal epithelium .
	manualset3
179330	2	413869	7	NULL	NULL	0	NULL	N-cadherin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that N-cadherin may be a critical cell-to-cell adhesion molecule between corneal epithelial stem/progenitor cells and their corresponding niche cells in the limbal epithelium .
	manualset3
179331	3	413869	7	NULL	NULL	0	NULL	cell-to-cell adhesion molecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that N-cadherin may be a critical cell-to-cell adhesion molecule between corneal epithelial stem/progenitor cells and their corresponding niche cells in the limbal epithelium .
	manualset3
179332	4	413869	7	NULL	NULL	0	NULL	corneal epithelial stem/progenitor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that N-cadherin may be a critical cell-to-cell adhesion molecule between corneal epithelial stem/progenitor cells and their corresponding niche cells in the limbal epithelium .
	manualset3
179333	5	413869	7	NULL	NULL	0	NULL	niche cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that N-cadherin may be a critical cell-to-cell adhesion molecule between corneal epithelial stem/progenitor cells and their corresponding niche cells in the limbal epithelium .
	manualset3
179334	6	413869	7	NULL	NULL	0	NULL	limbal epithelium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that N-cadherin may be a critical cell-to-cell adhesion molecule between corneal epithelial stem/progenitor cells and their corresponding niche cells in the limbal epithelium .
	manualset3
179335	1	413870	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that TP1 is likely to be an important parameter in the histone-to-protamine exchange and in the initiation of spermatid elongation .
	manualset3
179336	2	413870	7	NULL	NULL	0	NULL	TP1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that TP1 is likely to be an important parameter in the histone-to-protamine exchange and in the initiation of spermatid elongation .
	manualset3
179337	3	413870	7	NULL	NULL	0	NULL	parameter	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that TP1 is likely to be an important parameter in the histone-to-protamine exchange and in the initiation of spermatid elongation .
	manualset3
179338	4	413870	7	NULL	NULL	0	NULL	histone-to-protamine exchange	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that TP1 is likely to be an important parameter in the histone-to-protamine exchange and in the initiation of spermatid elongation .
	manualset3
179339	5	413870	7	NULL	NULL	0	NULL	initiation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that TP1 is likely to be an important parameter in the histone-to-protamine exchange and in the initiation of spermatid elongation .
	manualset3
179340	6	413870	7	NULL	NULL	0	NULL	spermatid elongation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that TP1 is likely to be an important parameter in the histone-to-protamine exchange and in the initiation of spermatid elongation .
	manualset3
179341	1	413871	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that TyDC5 expression is transcriptionally regulated and suggest that the TyDC5 enzyme may play an important role in providing precursors for alkaloid synthesis in the roots and germinating seedlings of opium poppy .
	manualset3
179342	2	413871	7	NULL	NULL	0	NULL	TyDC5 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that TyDC5 expression is transcriptionally regulated and suggest that the TyDC5 enzyme may play an important role in providing precursors for alkaloid synthesis in the roots and germinating seedlings of opium poppy .
	manualset3
179343	3	413871	7	NULL	NULL	0	NULL	TyDC5 enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that TyDC5 expression is transcriptionally regulated and suggest that the TyDC5 enzyme may play an important role in providing precursors for alkaloid synthesis in the roots and germinating seedlings of opium poppy .
	manualset3
179344	4	413871	7	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that TyDC5 expression is transcriptionally regulated and suggest that the TyDC5 enzyme may play an important role in providing precursors for alkaloid synthesis in the roots and germinating seedlings of opium poppy .
	manualset3
179345	5	413871	7	NULL	NULL	0	NULL	precursors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that TyDC5 expression is transcriptionally regulated and suggest that the TyDC5 enzyme may play an important role in providing precursors for alkaloid synthesis in the roots and germinating seedlings of opium poppy .
	manualset3
179346	6	413871	7	NULL	NULL	0	NULL	alkaloid synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that TyDC5 expression is transcriptionally regulated and suggest that the TyDC5 enzyme may play an important role in providing precursors for alkaloid synthesis in the roots and germinating seedlings of opium poppy .
	manualset3
179347	7	413871	7	NULL	NULL	0	NULL	roots	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that TyDC5 expression is transcriptionally regulated and suggest that the TyDC5 enzyme may play an important role in providing precursors for alkaloid synthesis in the roots and germinating seedlings of opium poppy .
	manualset3
179348	8	413871	7	NULL	NULL	0	NULL	germinating seedlings	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that TyDC5 expression is transcriptionally regulated and suggest that the TyDC5 enzyme may play an important role in providing precursors for alkaloid synthesis in the roots and germinating seedlings of opium poppy .
	manualset3
179349	9	413871	7	NULL	NULL	0	NULL	opium poppy	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that TyDC5 expression is transcriptionally regulated and suggest that the TyDC5 enzyme may play an important role in providing precursors for alkaloid synthesis in the roots and germinating seedlings of opium poppy .
	manualset3
179350	1	413872	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that c-erbB-2 or p53 expression is not significantly associated with tumor response to neo-adjuvant chemo/radiotherapy in our series of breast cancers .
	manualset3
179351	2	413872	7	NULL	NULL	0	NULL	c-erbB-2 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that c-erbB-2 or p53 expression is not significantly associated with tumor response to neo-adjuvant chemo/radiotherapy in our series of breast cancers .
	manualset3
179352	3	413872	7	NULL	NULL	0	NULL	p53 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that c-erbB-2 or p53 expression is not significantly associated with tumor response to neo-adjuvant chemo/radiotherapy in our series of breast cancers .
	manualset3
179353	4	413872	7	NULL	NULL	0	NULL	tumor response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that c-erbB-2 or p53 expression is not significantly associated with tumor response to neo-adjuvant chemo/radiotherapy in our series of breast cancers .
	manualset3
179354	5	413872	7	NULL	NULL	0	NULL	neo-adjuvant chemo/radiotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that c-erbB-2 or p53 expression is not significantly associated with tumor response to neo-adjuvant chemo/radiotherapy in our series of breast cancers .
	manualset3
179355	6	413872	7	NULL	NULL	NULL	NULL	series	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results indicate that c-erbB-2 or p53 expression is not significantly associated with tumor response to neo-adjuvant chemo/radiotherapy in our series of breast cancers .
	manualset3
179356	7	413872	7	NULL	NULL	0	NULL	breast cancers	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that c-erbB-2 or p53 expression is not significantly associated with tumor response to neo-adjuvant chemo/radiotherapy in our series of breast cancers .
	manualset3
179357	1	413873	7	NULL	NULL	0	NULL	Additional studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional studies showed that the interaction of HDAC1 with LIP provides for active repression of C/ebp transcription and is largely responsible for the ability of LIP and HDAC1 to repress preadipocyte differentiation .
	manualset3
179358	2	413873	7	NULL	NULL	0	NULL	 interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional studies showed that the interaction of HDAC1 with LIP provides for active repression of C/ebp transcription and is largely responsible for the ability of LIP and HDAC1 to repress preadipocyte differentiation .
	manualset3
179359	3	413873	7	NULL	NULL	0	NULL	HDAC1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional studies showed that the interaction of HDAC1 with LIP provides for active repression of C/ebp transcription and is largely responsible for the ability of LIP and HDAC1 to repress preadipocyte differentiation .
	manualset3
179360	4	413873	7	NULL	NULL	0	NULL	LIP 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional studies showed that the interaction of HDAC1 with LIP provides for active repression of C/ebp transcription and is largely responsible for the ability of LIP and HDAC1 to repress preadipocyte differentiation .
	manualset3
179361	5	413873	7	NULL	NULL	0	NULL	active repression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional studies showed that the interaction of HDAC1 with LIP provides for active repression of C/ebp transcription and is largely responsible for the ability of LIP and HDAC1 to repress preadipocyte differentiation .
	manualset3
179362	6	413873	7	NULL	NULL	0	NULL	C/ebp transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional studies showed that the interaction of HDAC1 with LIP provides for active repression of C/ebp transcription and is largely responsible for the ability of LIP and HDAC1 to repress preadipocyte differentiation .
	manualset3
179363	7	413873	7	NULL	NULL	0	NULL	ability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional studies showed that the interaction of HDAC1 with LIP provides for active repression of C/ebp transcription and is largely responsible for the ability of LIP and HDAC1 to repress preadipocyte differentiation .
	manualset3
179364	8	413873	7	NULL	NULL	0	NULL	LIP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional studies showed that the interaction of HDAC1 with LIP provides for active repression of C/ebp transcription and is largely responsible for the ability of LIP and HDAC1 to repress preadipocyte differentiation .
	manualset3
179365	9	413873	7	NULL	NULL	0	NULL	HDAC1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional studies showed that the interaction of HDAC1 with LIP provides for active repression of C/ebp transcription and is largely responsible for the ability of LIP and HDAC1 to repress preadipocyte differentiation .
	manualset3
179366	10	413873	7	NULL	NULL	0	NULL	preadipocyte differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional studies showed that the interaction of HDAC1 with LIP provides for active repression of C/ebp transcription and is largely responsible for the ability of LIP and HDAC1 to repress preadipocyte differentiation .
	manualset3
179367	1	413874	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that genotype , age , salt type , and salt concentration can interact to influence salt preference in hypertension .
	manualset3
179368	2	413874	7	NULL	NULL	NULL	NULL	genotype	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results indicate that genotype , age , salt type , and salt concentration can interact to influence salt preference in hypertension .
	manualset3
179369	3	413874	7	NULL	NULL	0	NULL	age	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that genotype , age , salt type , and salt concentration can interact to influence salt preference in hypertension .
	manualset3
179370	4	413874	7	NULL	NULL	0	NULL	salt type	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that genotype , age , salt type , and salt concentration can interact to influence salt preference in hypertension .
	manualset3
179371	5	413874	7	NULL	NULL	0	NULL	salt concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that genotype , age , salt type , and salt concentration can interact to influence salt preference in hypertension .
	manualset3
179372	6	413874	7	NULL	NULL	0	NULL	salt preference	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that genotype , age , salt type , and salt concentration can interact to influence salt preference in hypertension .
	manualset3
179373	7	413874	7	NULL	NULL	0	NULL	hypertension 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that genotype , age , salt type , and salt concentration can interact to influence salt preference in hypertension .
	manualset3
179374	1	413875	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that intranasal delivery of mouse ( D-Leu-4 ) OB3 with Intravail is a more effective method of peptide administration than injection methods , and suggest that it may have potential as a novel , non-invasive approach to the treatment of obesity and its associated metabolic dysfunctions in humans .
	manualset3
179375	2	413875	7	NULL	NULL	0	NULL	intranasal delivery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that intranasal delivery of mouse ( D-Leu-4 ) OB3 with Intravail is a more effective method of peptide administration than injection methods , and suggest that it may have potential as a novel , non-invasive approach to the treatment of obesity and its associated metabolic dysfunctions in humans .
	manualset3
179376	3	413875	7	NULL	NULL	0	NULL	mouse ( D-Leu-4 ) OB3	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that intranasal delivery of mouse ( D-Leu-4 ) OB3 with Intravail is a more effective method of peptide administration than injection methods , and suggest that it may have potential as a novel , non-invasive approach to the treatment of obesity and its associated metabolic dysfunctions in humans .
	manualset3
179377	4	413875	7	NULL	NULL	0	NULL	Intravail	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that intranasal delivery of mouse ( D-Leu-4 ) OB3 with Intravail is a more effective method of peptide administration than injection methods , and suggest that it may have potential as a novel , non-invasive approach to the treatment of obesity and its associated metabolic dysfunctions in humans .
	manualset3
179378	5	413875	7	NULL	NULL	0	NULL	effective method	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that intranasal delivery of mouse ( D-Leu-4 ) OB3 with Intravail is a more effective method of peptide administration than injection methods , and suggest that it may have potential as a novel , non-invasive approach to the treatment of obesity and its associated metabolic dysfunctions in humans .
	manualset3
179379	6	413875	7	NULL	NULL	0	NULL	peptide administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that intranasal delivery of mouse ( D-Leu-4 ) OB3 with Intravail is a more effective method of peptide administration than injection methods , and suggest that it may have potential as a novel , non-invasive approach to the treatment of obesity and its associated metabolic dysfunctions in humans .
	manualset3
179380	7	413875	7	NULL	NULL	0	NULL	 injection methods	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that intranasal delivery of mouse ( D-Leu-4 ) OB3 with Intravail is a more effective method of peptide administration than injection methods , and suggest that it may have potential as a novel , non-invasive approach to the treatment of obesity and its associated metabolic dysfunctions in humans .
	manualset3
179381	8	413875	7	NULL	NULL	0	NULL	novel , non-invasive approach	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that intranasal delivery of mouse ( D-Leu-4 ) OB3 with Intravail is a more effective method of peptide administration than injection methods , and suggest that it may have potential as a novel , non-invasive approach to the treatment of obesity and its associated metabolic dysfunctions in humans .
	manualset3
179382	9	413875	7	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that intranasal delivery of mouse ( D-Leu-4 ) OB3 with Intravail is a more effective method of peptide administration than injection methods , and suggest that it may have potential as a novel , non-invasive approach to the treatment of obesity and its associated metabolic dysfunctions in humans .
	manualset3
179383	10	413875	7	NULL	NULL	0	NULL	obesity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that intranasal delivery of mouse ( D-Leu-4 ) OB3 with Intravail is a more effective method of peptide administration than injection methods , and suggest that it may have potential as a novel , non-invasive approach to the treatment of obesity and its associated metabolic dysfunctions in humans .
	manualset3
179384	11	413875	7	NULL	NULL	NULL	NULL	metabolic dysfunctions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results indicate that intranasal delivery of mouse ( D-Leu-4 ) OB3 with Intravail is a more effective method of peptide administration than injection methods , and suggest that it may have potential as a novel , non-invasive approach to the treatment of obesity and its associated metabolic dysfunctions in humans .
	manualset3
179385	12	413875	7	NULL	NULL	0	NULL	humans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that intranasal delivery of mouse ( D-Leu-4 ) OB3 with Intravail is a more effective method of peptide administration than injection methods , and suggest that it may have potential as a novel , non-invasive approach to the treatment of obesity and its associated metabolic dysfunctions in humans .
	manualset3
179386	1	413876	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that nicotine administration during the ethanol deprivation period can exacerbate the maintenance of alcohol consumption .
	manualset3
179387	2	413876	7	NULL	NULL	0	NULL	nicotine administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that nicotine administration during the ethanol deprivation period can exacerbate the maintenance of alcohol consumption .
	manualset3
179388	3	413876	7	NULL	NULL	0	NULL	ethanol deprivation period	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that nicotine administration during the ethanol deprivation period can exacerbate the maintenance of alcohol consumption .
	manualset3
179389	4	413876	7	NULL	NULL	0	NULL	maintenance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that nicotine administration during the ethanol deprivation period can exacerbate the maintenance of alcohol consumption .
	manualset3
179390	5	413876	7	NULL	NULL	0	NULL	alcohol consumption	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that nicotine administration during the ethanol deprivation period can exacerbate the maintenance of alcohol consumption .
	manualset3
179391	1	413877	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that sole enhancement of XIAP or Bcl-xL is not sufficient to counteract QA-induced excitotoxic insult of striatal neurons .
	manualset3
179392	2	413877	7	NULL	NULL	0	NULL	enhancement	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that sole enhancement of XIAP or Bcl-xL is not sufficient to counteract QA-induced excitotoxic insult of striatal neurons .
	manualset3
179393	3	413877	7	NULL	NULL	0	NULL	XIAP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that sole enhancement of XIAP or Bcl-xL is not sufficient to counteract QA-induced excitotoxic insult of striatal neurons .
	manualset3
179394	4	413877	7	NULL	NULL	0	NULL	Bcl-xL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that sole enhancement of XIAP or Bcl-xL is not sufficient to counteract QA-induced excitotoxic insult of striatal neurons .
	manualset3
179395	5	413877	7	NULL	NULL	0	NULL	QA-induced excitotoxic insult	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that sole enhancement of XIAP or Bcl-xL is not sufficient to counteract QA-induced excitotoxic insult of striatal neurons .
	manualset3
179396	6	413877	7	NULL	NULL	0	NULL	striatal neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that sole enhancement of XIAP or Bcl-xL is not sufficient to counteract QA-induced excitotoxic insult of striatal neurons .
	manualset3
179397	1	413878	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the J-T hg of mt-DNA may have a modulator effect on deeper determinants of schizophrenia .
	manualset3
179398	2	413878	7	NULL	NULL	0	NULL	J-T hg	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the J-T hg of mt-DNA may have a modulator effect on deeper determinants of schizophrenia .
	manualset3
179399	3	413878	7	NULL	NULL	0	NULL	 mt-DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the J-T hg of mt-DNA may have a modulator effect on deeper determinants of schizophrenia .
	manualset3
179400	4	413878	7	NULL	NULL	0	NULL	modulator effect 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the J-T hg of mt-DNA may have a modulator effect on deeper determinants of schizophrenia .
	manualset3
179401	5	413878	7	NULL	NULL	0	NULL	deeper determinants	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the J-T hg of mt-DNA may have a modulator effect on deeper determinants of schizophrenia .
	manualset3
179402	6	413878	7	NULL	NULL	0	NULL	schizophrenia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the J-T hg of mt-DNA may have a modulator effect on deeper determinants of schizophrenia .
	manualset3
179403	1	413879	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the SA reflects feature-level perceptual grouping , not emotional valence .
	manualset3
179404	2	413879	7	NULL	NULL	0	NULL	SA	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the SA reflects feature-level perceptual grouping , not emotional valence .
	manualset3
179405	3	413879	7	NULL	NULL	0	NULL	 feature-level perceptual grouping	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the SA reflects feature-level perceptual grouping , not emotional valence .
	manualset3
179406	4	413879	7	NULL	NULL	0	NULL	emotional valence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the SA reflects feature-level perceptual grouping , not emotional valence .
	manualset3
179407	1	413880	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the beta-blocker pindolol has vasodilatory properties owing to stimulation of vascular beta 2-adrenergic receptors and that this effect may be of therapeutic relevance .
	manualset3
179408	2	413880	7	NULL	NULL	0	NULL	beta-blocker pindolol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the beta-blocker pindolol has vasodilatory properties owing to stimulation of vascular beta 2-adrenergic receptors and that this effect may be of therapeutic relevance .
	manualset3
179409	3	413880	7	NULL	NULL	0	NULL	vasodilatory properties	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the beta-blocker pindolol has vasodilatory properties owing to stimulation of vascular beta 2-adrenergic receptors and that this effect may be of therapeutic relevance .
	manualset3
179410	4	413880	7	NULL	NULL	0	NULL	stimulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the beta-blocker pindolol has vasodilatory properties owing to stimulation of vascular beta 2-adrenergic receptors and that this effect may be of therapeutic relevance .
	manualset3
179411	5	413880	7	NULL	NULL	0	NULL	vascular beta 2-adrenergic receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the beta-blocker pindolol has vasodilatory properties owing to stimulation of vascular beta 2-adrenergic receptors and that this effect may be of therapeutic relevance .
	manualset3
179412	6	413880	7	NULL	NULL	0	NULL	effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the beta-blocker pindolol has vasodilatory properties owing to stimulation of vascular beta 2-adrenergic receptors and that this effect may be of therapeutic relevance .
	manualset3
179413	7	413880	7	NULL	NULL	0	NULL	therapeutic relevance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the beta-blocker pindolol has vasodilatory properties owing to stimulation of vascular beta 2-adrenergic receptors and that this effect may be of therapeutic relevance .
	manualset3
179414	1	413881	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the co-culture microenvironment plays a decisive role for the hepatic differentiation of MSCs , and it is more efficient than HGF treatment .
	manualset3
179415	2	413881	7	NULL	NULL	0	NULL	 co-culture microenvironment	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the co-culture microenvironment plays a decisive role for the hepatic differentiation of MSCs , and it is more efficient than HGF treatment .
	manualset3
179416	3	413881	7	NULL	NULL	0	NULL	decisive role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the co-culture microenvironment plays a decisive role for the hepatic differentiation of MSCs , and it is more efficient than HGF treatment .
	manualset3
179417	4	413881	7	NULL	NULL	0	NULL	hepatic differentiation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the co-culture microenvironment plays a decisive role for the hepatic differentiation of MSCs , and it is more efficient than HGF treatment .
	manualset3
179418	5	413881	7	NULL	NULL	0	NULL	MSCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the co-culture microenvironment plays a decisive role for the hepatic differentiation of MSCs , and it is more efficient than HGF treatment .
	manualset3
179419	6	413881	7	NULL	NULL	0	NULL	HGF treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the co-culture microenvironment plays a decisive role for the hepatic differentiation of MSCs , and it is more efficient than HGF treatment .
	manualset3
179420	1	413882	7	NULL	NULL	NULL	NULL	substitution mapping	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Additional substitution mapping located the QTL to & lt ; 0.4 cM or approximately 493 kb .
	manualset3
179421	2	413882	7	NULL	NULL	0	NULL	QTL	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional substitution mapping located the QTL to & lt ; 0.4 cM or approximately 493 kb .
	manualset3
179422	3	413882	7	NULL	NULL	NULL	NULL	& lt ; 0.4 cM	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Additional substitution mapping located the QTL to & lt ; 0.4 cM or approximately 493 kb .
	manualset3
179423	4	413882	7	NULL	NULL	0	NULL	 493 kb	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional substitution mapping located the QTL to & lt ; 0.4 cM or approximately 493 kb .
	manualset3
179424	1	413883	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the female reproductive cycle is an important variable in basal blood volume regulation and in plasma protein and plasma volume restitution following blood loss .
	manualset3
179425	2	413883	7	NULL	NULL	0	NULL	female reproductive cycle	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the female reproductive cycle is an important variable in basal blood volume regulation and in plasma protein and plasma volume restitution following blood loss .
	manualset3
179426	3	413883	7	NULL	NULL	0	NULL	variable	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the female reproductive cycle is an important variable in basal blood volume regulation and in plasma protein and plasma volume restitution following blood loss .
	manualset3
179427	4	413883	7	NULL	NULL	0	NULL	basal blood volume regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the female reproductive cycle is an important variable in basal blood volume regulation and in plasma protein and plasma volume restitution following blood loss .
	manualset3
179428	5	413883	7	NULL	NULL	0	NULL	plasma protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the female reproductive cycle is an important variable in basal blood volume regulation and in plasma protein and plasma volume restitution following blood loss .
	manualset3
179429	6	413883	7	NULL	NULL	0	NULL	 plasma volume restitution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the female reproductive cycle is an important variable in basal blood volume regulation and in plasma protein and plasma volume restitution following blood loss .
	manualset3
179430	7	413883	7	NULL	NULL	0	NULL	blood loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the female reproductive cycle is an important variable in basal blood volume regulation and in plasma protein and plasma volume restitution following blood loss .
	manualset3
179431	1	413884	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the inability to degrade DNA derived from erythroid precursors results in interferon-beta production that induces expression of a specific set of interferon-responsive genes associated with embryonic lethality in DNase II-deficient mice .
	manualset3
179432	2	413884	7	NULL	NULL	0	NULL	 inability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the inability to degrade DNA derived from erythroid precursors results in interferon-beta production that induces expression of a specific set of interferon-responsive genes associated with embryonic lethality in DNase II-deficient mice .
	manualset3
179433	3	413884	7	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the inability to degrade DNA derived from erythroid precursors results in interferon-beta production that induces expression of a specific set of interferon-responsive genes associated with embryonic lethality in DNase II-deficient mice .
	manualset3
179434	4	413884	7	NULL	NULL	0	NULL	erythroid precursors 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the inability to degrade DNA derived from erythroid precursors results in interferon-beta production that induces expression of a specific set of interferon-responsive genes associated with embryonic lethality in DNase II-deficient mice .
	manualset3
179435	5	413884	7	NULL	NULL	0	NULL	interferon-beta production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the inability to degrade DNA derived from erythroid precursors results in interferon-beta production that induces expression of a specific set of interferon-responsive genes associated with embryonic lethality in DNase II-deficient mice .
	manualset3
179436	6	413884	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the inability to degrade DNA derived from erythroid precursors results in interferon-beta production that induces expression of a specific set of interferon-responsive genes associated with embryonic lethality in DNase II-deficient mice .
	manualset3
179437	7	413884	7	NULL	NULL	0	NULL	set	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the inability to degrade DNA derived from erythroid precursors results in interferon-beta production that induces expression of a specific set of interferon-responsive genes associated with embryonic lethality in DNase II-deficient mice .
	manualset3
179438	8	413884	7	NULL	NULL	0	NULL	interferon-responsive genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the inability to degrade DNA derived from erythroid precursors results in interferon-beta production that induces expression of a specific set of interferon-responsive genes associated with embryonic lethality in DNase II-deficient mice .
	manualset3
179439	9	413884	7	NULL	NULL	0	NULL	embryonic lethality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the inability to degrade DNA derived from erythroid precursors results in interferon-beta production that induces expression of a specific set of interferon-responsive genes associated with embryonic lethality in DNase II-deficient mice .
	manualset3
179440	10	413884	7	NULL	NULL	0	NULL	DNase II-deficient mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the inability to degrade DNA derived from erythroid precursors results in interferon-beta production that induces expression of a specific set of interferon-responsive genes associated with embryonic lethality in DNase II-deficient mice .
	manualset3
179441	1	413885	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the present internal radiolabelling procedure does not alter the ability of the monoclonal antibody to recognize the endogenous antigen .
	manualset3
179442	2	413885	7	NULL	NULL	0	NULL	internal radiolabelling procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the present internal radiolabelling procedure does not alter the ability of the monoclonal antibody to recognize the endogenous antigen .
	manualset3
179443	3	413885	7	NULL	NULL	0	NULL	ability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the present internal radiolabelling procedure does not alter the ability of the monoclonal antibody to recognize the endogenous antigen .
	manualset3
179444	4	413885	7	NULL	NULL	0	NULL	monoclonal antibody	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the present internal radiolabelling procedure does not alter the ability of the monoclonal antibody to recognize the endogenous antigen .
	manualset3
179445	5	413885	7	NULL	NULL	0	NULL	endogenous antigen	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that the present internal radiolabelling procedure does not alter the ability of the monoclonal antibody to recognize the endogenous antigen .
	manualset3
179446	1	413886	7	NULL	NULL	0	NULL	 results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that under these conditions tocopherol is a major reducing agent in LDL , converting Cu2 + to Cu + , and therefore , may play an important role in promoting LDL oxidation .
	manualset3
179447	2	413886	7	NULL	NULL	0	NULL	conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that under these conditions tocopherol is a major reducing agent in LDL , converting Cu2 + to Cu + , and therefore , may play an important role in promoting LDL oxidation .
	manualset3
179448	3	413886	7	NULL	NULL	0	NULL	tocopherol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that under these conditions tocopherol is a major reducing agent in LDL , converting Cu2 + to Cu + , and therefore , may play an important role in promoting LDL oxidation .
	manualset3
179449	4	413886	7	NULL	NULL	0	NULL	reducing agent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that under these conditions tocopherol is a major reducing agent in LDL , converting Cu2 + to Cu + , and therefore , may play an important role in promoting LDL oxidation .
	manualset3
179450	5	413886	7	NULL	NULL	0	NULL	LDL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that under these conditions tocopherol is a major reducing agent in LDL , converting Cu2 + to Cu + , and therefore , may play an important role in promoting LDL oxidation .
	manualset3
179451	6	413886	7	NULL	NULL	0	NULL	Cu2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that under these conditions tocopherol is a major reducing agent in LDL , converting Cu2 + to Cu + , and therefore , may play an important role in promoting LDL oxidation .
	manualset3
179452	7	413886	7	NULL	NULL	0	NULL	Cu +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that under these conditions tocopherol is a major reducing agent in LDL , converting Cu2 + to Cu + , and therefore , may play an important role in promoting LDL oxidation .
	manualset3
179453	8	413886	7	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that under these conditions tocopherol is a major reducing agent in LDL , converting Cu2 + to Cu + , and therefore , may play an important role in promoting LDL oxidation .
	manualset3
179454	9	413886	7	NULL	NULL	0	NULL	LDL oxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that under these conditions tocopherol is a major reducing agent in LDL , converting Cu2 + to Cu + , and therefore , may play an important role in promoting LDL oxidation .
	manualset3
179455	1	413887	7	NULL	NULL	0	NULL	 results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that uremic children on hemodialysis have similar lipid and apolipoprotein abnormalities to those found in adults who may have a risk of cardiovascular disease .
	manualset3
179456	2	413887	7	NULL	NULL	0	NULL	uremic children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that uremic children on hemodialysis have similar lipid and apolipoprotein abnormalities to those found in adults who may have a risk of cardiovascular disease .
	manualset3
179457	3	413887	7	NULL	NULL	0	NULL	hemodialysis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that uremic children on hemodialysis have similar lipid and apolipoprotein abnormalities to those found in adults who may have a risk of cardiovascular disease .
	manualset3
179458	4	413887	7	NULL	NULL	0	NULL	 lipid abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that uremic children on hemodialysis have similar lipid and apolipoprotein abnormalities to those found in adults who may have a risk of cardiovascular disease .
	manualset3
179459	5	413887	7	NULL	NULL	0	NULL	apolipoprotein abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that uremic children on hemodialysis have similar lipid and apolipoprotein abnormalities to those found in adults who may have a risk of cardiovascular disease .
	manualset3
179460	6	413887	7	NULL	NULL	0	NULL	adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that uremic children on hemodialysis have similar lipid and apolipoprotein abnormalities to those found in adults who may have a risk of cardiovascular disease .
	manualset3
179461	7	413887	7	NULL	NULL	0	NULL	 risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that uremic children on hemodialysis have similar lipid and apolipoprotein abnormalities to those found in adults who may have a risk of cardiovascular disease .
	manualset3
179462	8	413887	7	NULL	NULL	0	NULL	cardiovascular disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicate that uremic children on hemodialysis have similar lipid and apolipoprotein abnormalities to those found in adults who may have a risk of cardiovascular disease .
	manualset3
179463	1	413888	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicated that CYP and several conjugation enzymes participate in its biotransformation , and sulfation is important in D. magna for metabolism and elimination of xenobiotics .
	manualset3
179464	2	413888	7	NULL	NULL	0	NULL	 CYP	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicated that CYP and several conjugation enzymes participate in its biotransformation , and sulfation is important in D. magna for metabolism and elimination of xenobiotics .
	manualset3
179465	3	413888	7	NULL	NULL	0	NULL	conjugation enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicated that CYP and several conjugation enzymes participate in its biotransformation , and sulfation is important in D. magna for metabolism and elimination of xenobiotics .
	manualset3
179466	4	413888	7	NULL	NULL	0	NULL	biotransformation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicated that CYP and several conjugation enzymes participate in its biotransformation , and sulfation is important in D. magna for metabolism and elimination of xenobiotics .
	manualset3
179467	5	413888	7	NULL	NULL	0	NULL	sulfation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicated that CYP and several conjugation enzymes participate in its biotransformation , and sulfation is important in D. magna for metabolism and elimination of xenobiotics .
	manualset3
179468	6	413888	7	NULL	NULL	0	NULL	D. magna	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicated that CYP and several conjugation enzymes participate in its biotransformation , and sulfation is important in D. magna for metabolism and elimination of xenobiotics .
	manualset3
179469	7	413888	7	NULL	NULL	0	NULL	metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicated that CYP and several conjugation enzymes participate in its biotransformation , and sulfation is important in D. magna for metabolism and elimination of xenobiotics .
	manualset3
179470	8	413888	7	NULL	NULL	0	NULL	elimination	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicated that CYP and several conjugation enzymes participate in its biotransformation , and sulfation is important in D. magna for metabolism and elimination of xenobiotics .
	manualset3
179471	9	413888	7	NULL	NULL	0	NULL	xenobiotics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results indicated that CYP and several conjugation enzymes participate in its biotransformation , and sulfation is important in D. magna for metabolism and elimination of xenobiotics .
	manualset3
179472	1	413889	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results may contribute to explain the importance of Abeta alone or in the presence of redox-available iron in association with Abeta plaques ( and neurofibrillary tangles ) in AD brains and the significant role played by H2O2 as a second messenger of death signal in some degenerative diseases linked to oxidative stress stimuli .
	manualset3
179473	2	413889	7	NULL	NULL	0	NULL	Abeta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results may contribute to explain the importance of Abeta alone or in the presence of redox-available iron in association with Abeta plaques ( and neurofibrillary tangles ) in AD brains and the significant role played by H2O2 as a second messenger of death signal in some degenerative diseases linked to oxidative stress stimuli .
	manualset3
179474	3	413889	7	NULL	NULL	0	NULL	presence	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results may contribute to explain the importance of Abeta alone or in the presence of redox-available iron in association with Abeta plaques ( and neurofibrillary tangles ) in AD brains and the significant role played by H2O2 as a second messenger of death signal in some degenerative diseases linked to oxidative stress stimuli .
	manualset3
179475	4	413889	7	NULL	NULL	0	NULL	redox-available iron	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results may contribute to explain the importance of Abeta alone or in the presence of redox-available iron in association with Abeta plaques ( and neurofibrillary tangles ) in AD brains and the significant role played by H2O2 as a second messenger of death signal in some degenerative diseases linked to oxidative stress stimuli .
	manualset3
179476	5	413889	7	NULL	NULL	0	NULL	association	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results may contribute to explain the importance of Abeta alone or in the presence of redox-available iron in association with Abeta plaques ( and neurofibrillary tangles ) in AD brains and the significant role played by H2O2 as a second messenger of death signal in some degenerative diseases linked to oxidative stress stimuli .
	manualset3
179477	6	413889	7	NULL	NULL	NULL	NULL	Abeta plaques	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results may contribute to explain the importance of Abeta alone or in the presence of redox-available iron in association with Abeta plaques ( and neurofibrillary tangles ) in AD brains and the significant role played by H2O2 as a second messenger of death signal in some degenerative diseases linked to oxidative stress stimuli .
	manualset3
179478	7	413889	7	NULL	NULL	0	NULL	neurofibrillary tangles	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results may contribute to explain the importance of Abeta alone or in the presence of redox-available iron in association with Abeta plaques ( and neurofibrillary tangles ) in AD brains and the significant role played by H2O2 as a second messenger of death signal in some degenerative diseases linked to oxidative stress stimuli .
	manualset3
179479	8	413889	7	NULL	NULL	0	NULL	AD brains 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results may contribute to explain the importance of Abeta alone or in the presence of redox-available iron in association with Abeta plaques ( and neurofibrillary tangles ) in AD brains and the significant role played by H2O2 as a second messenger of death signal in some degenerative diseases linked to oxidative stress stimuli .
	manualset3
179480	9	413889	7	NULL	NULL	0	NULL	 role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results may contribute to explain the importance of Abeta alone or in the presence of redox-available iron in association with Abeta plaques ( and neurofibrillary tangles ) in AD brains and the significant role played by H2O2 as a second messenger of death signal in some degenerative diseases linked to oxidative stress stimuli .
	manualset3
179481	10	413889	7	NULL	NULL	0	NULL	H2O2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results may contribute to explain the importance of Abeta alone or in the presence of redox-available iron in association with Abeta plaques ( and neurofibrillary tangles ) in AD brains and the significant role played by H2O2 as a second messenger of death signal in some degenerative diseases linked to oxidative stress stimuli .
	manualset3
179482	11	413889	7	NULL	NULL	0	NULL	second messenger 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results may contribute to explain the importance of Abeta alone or in the presence of redox-available iron in association with Abeta plaques ( and neurofibrillary tangles ) in AD brains and the significant role played by H2O2 as a second messenger of death signal in some degenerative diseases linked to oxidative stress stimuli .
	manualset3
179483	12	413889	7	NULL	NULL	NULL	NULL	death signal	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results may contribute to explain the importance of Abeta alone or in the presence of redox-available iron in association with Abeta plaques ( and neurofibrillary tangles ) in AD brains and the significant role played by H2O2 as a second messenger of death signal in some degenerative diseases linked to oxidative stress stimuli .
	manualset3
179484	13	413889	7	NULL	NULL	0	NULL	degenerative diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results may contribute to explain the importance of Abeta alone or in the presence of redox-available iron in association with Abeta plaques ( and neurofibrillary tangles ) in AD brains and the significant role played by H2O2 as a second messenger of death signal in some degenerative diseases linked to oxidative stress stimuli .
	manualset3
179485	14	413889	7	NULL	NULL	0	NULL	 oxidative stress stimuli	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results may contribute to explain the importance of Abeta alone or in the presence of redox-available iron in association with Abeta plaques ( and neurofibrillary tangles ) in AD brains and the significant role played by H2O2 as a second messenger of death signal in some degenerative diseases linked to oxidative stress stimuli .
	manualset3
179486	1	413890	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results may facilitate not only using the molecular marker assisted selection of PTGMS genes , but also cloning of the pms1 ( t ) gene itself .
	manualset3
179487	2	413890	7	NULL	NULL	NULL	NULL	molecular marker assisted selection	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results may facilitate not only using the molecular marker assisted selection of PTGMS genes , but also cloning of the pms1 ( t ) gene itself .
	manualset3
179488	3	413890	7	NULL	NULL	0	NULL	PTGMS genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	These results may facilitate not only using the molecular marker assisted selection of PTGMS genes , but also cloning of the pms1 ( t ) gene itself .
	manualset3
179489	4	413890	7	NULL	NULL	0	NULL	cloning	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results may facilitate not only using the molecular marker assisted selection of PTGMS genes , but also cloning of the pms1 ( t ) gene itself .
	manualset3
179490	5	413890	7	NULL	NULL	0	NULL	pms1 ( t ) gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	These results may facilitate not only using the molecular marker assisted selection of PTGMS genes , but also cloning of the pms1 ( t ) gene itself .
	manualset3
179491	1	413891	7	NULL	NULL	0	NULL	Additional support	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional support for a modulatory role for ORL-1 receptors in buprenorphine-induced antinociception was that coadministration of J-113397 , an ORL-1 receptor antagonist , enhanced the antinociceptive efficacy of buprenorphine in wild-type mice but not in mice lacking ORL-1 receptors .
	manualset3
179492	2	413891	7	NULL	NULL	0	NULL	modulatory role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional support for a modulatory role for ORL-1 receptors in buprenorphine-induced antinociception was that coadministration of J-113397 , an ORL-1 receptor antagonist , enhanced the antinociceptive efficacy of buprenorphine in wild-type mice but not in mice lacking ORL-1 receptors .
	manualset3
179493	3	413891	7	NULL	NULL	0	NULL	ORL-1 receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional support for a modulatory role for ORL-1 receptors in buprenorphine-induced antinociception was that coadministration of J-113397 , an ORL-1 receptor antagonist , enhanced the antinociceptive efficacy of buprenorphine in wild-type mice but not in mice lacking ORL-1 receptors .
	manualset3
179494	4	413891	7	NULL	NULL	NULL	NULL	buprenorphine-induced antinociception	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Additional support for a modulatory role for ORL-1 receptors in buprenorphine-induced antinociception was that coadministration of J-113397 , an ORL-1 receptor antagonist , enhanced the antinociceptive efficacy of buprenorphine in wild-type mice but not in mice lacking ORL-1 receptors .
	manualset3
179495	5	413891	7	NULL	NULL	0	NULL	coadministration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional support for a modulatory role for ORL-1 receptors in buprenorphine-induced antinociception was that coadministration of J-113397 , an ORL-1 receptor antagonist , enhanced the antinociceptive efficacy of buprenorphine in wild-type mice but not in mice lacking ORL-1 receptors .
	manualset3
179496	6	413891	7	NULL	NULL	NULL	NULL	J-113397	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Additional support for a modulatory role for ORL-1 receptors in buprenorphine-induced antinociception was that coadministration of J-113397 , an ORL-1 receptor antagonist , enhanced the antinociceptive efficacy of buprenorphine in wild-type mice but not in mice lacking ORL-1 receptors .
	manualset3
179497	7	413891	7	NULL	NULL	0	NULL	ORL-1 receptor antagonist	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional support for a modulatory role for ORL-1 receptors in buprenorphine-induced antinociception was that coadministration of J-113397 , an ORL-1 receptor antagonist , enhanced the antinociceptive efficacy of buprenorphine in wild-type mice but not in mice lacking ORL-1 receptors .
	manualset3
179498	8	413891	7	NULL	NULL	0	NULL	antinociceptive efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional support for a modulatory role for ORL-1 receptors in buprenorphine-induced antinociception was that coadministration of J-113397 , an ORL-1 receptor antagonist , enhanced the antinociceptive efficacy of buprenorphine in wild-type mice but not in mice lacking ORL-1 receptors .
	manualset3
179499	9	413891	7	NULL	NULL	0	NULL	 buprenorphine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional support for a modulatory role for ORL-1 receptors in buprenorphine-induced antinociception was that coadministration of J-113397 , an ORL-1 receptor antagonist , enhanced the antinociceptive efficacy of buprenorphine in wild-type mice but not in mice lacking ORL-1 receptors .
	manualset3
179500	10	413891	7	NULL	NULL	0	NULL	wild-type mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional support for a modulatory role for ORL-1 receptors in buprenorphine-induced antinociception was that coadministration of J-113397 , an ORL-1 receptor antagonist , enhanced the antinociceptive efficacy of buprenorphine in wild-type mice but not in mice lacking ORL-1 receptors .
	manualset3
179501	11	413891	7	NULL	NULL	NULL	NULL	mice lacking ORL-1 receptors	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Additional support for a modulatory role for ORL-1 receptors in buprenorphine-induced antinociception was that coadministration of J-113397 , an ORL-1 receptor antagonist , enhanced the antinociceptive efficacy of buprenorphine in wild-type mice but not in mice lacking ORL-1 receptors .
	manualset3
179502	1	413892	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results may have implications for dental pulp development and regeneration .
	manualset3
179503	2	413892	7	NULL	NULL	0	NULL	implications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results may have implications for dental pulp development and regeneration .
	manualset3
179504	3	413892	7	NULL	NULL	NULL	NULL	dental pulp development	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results may have implications for dental pulp development and regeneration .
	manualset3
179505	4	413892	7	NULL	NULL	NULL	NULL	regeneration	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results may have implications for dental pulp development and regeneration .
	manualset3
179506	1	413893	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results may have implications for the pathophysiology and clinical management of ischemic retinal conditions .
	manualset3
179507	2	413893	7	NULL	NULL	0	NULL	 implications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results may have implications for the pathophysiology and clinical management of ischemic retinal conditions .
	manualset3
179508	3	413893	7	NULL	NULL	0	NULL	 pathophysiology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results may have implications for the pathophysiology and clinical management of ischemic retinal conditions .
	manualset3
179509	4	413893	7	NULL	NULL	0	NULL	clinical management	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results may have implications for the pathophysiology and clinical management of ischemic retinal conditions .
	manualset3
179510	5	413893	7	NULL	NULL	NULL	NULL	ischemic retinal conditions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results may have implications for the pathophysiology and clinical management of ischemic retinal conditions .
	manualset3
179695	1	413894	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results point to a neuroprotective role for GM1 and its associated exchanger in the nucleus , based on regulation of Ca2 + flux between nucleoplasm and nuclear envelope .
	manualset3
179696	2	413894	7	NULL	NULL	0	NULL	neuroprotective role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results point to a neuroprotective role for GM1 and its associated exchanger in the nucleus , based on regulation of Ca2 + flux between nucleoplasm and nuclear envelope .
	manualset3
179697	3	413894	7	NULL	NULL	0	NULL	GM1	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results point to a neuroprotective role for GM1 and its associated exchanger in the nucleus , based on regulation of Ca2 + flux between nucleoplasm and nuclear envelope .
	manualset3
179698	4	413894	7	NULL	NULL	0	NULL	exchanger	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results point to a neuroprotective role for GM1 and its associated exchanger in the nucleus , based on regulation of Ca2 + flux between nucleoplasm and nuclear envelope .
	manualset3
179699	5	413894	7	NULL	NULL	0	NULL	 nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These results point to a neuroprotective role for GM1 and its associated exchanger in the nucleus , based on regulation of Ca2 + flux between nucleoplasm and nuclear envelope .
	manualset3
179700	6	413894	7	NULL	NULL	0	NULL	regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results point to a neuroprotective role for GM1 and its associated exchanger in the nucleus , based on regulation of Ca2 + flux between nucleoplasm and nuclear envelope .
	manualset3
179701	7	413894	7	NULL	NULL	0	NULL	Ca2 + flux	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results point to a neuroprotective role for GM1 and its associated exchanger in the nucleus , based on regulation of Ca2 + flux between nucleoplasm and nuclear envelope .
	manualset3
179702	8	413894	7	NULL	NULL	0	NULL	nucleoplasm	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These results point to a neuroprotective role for GM1 and its associated exchanger in the nucleus , based on regulation of Ca2 + flux between nucleoplasm and nuclear envelope .
	manualset3
179703	9	413894	7	NULL	NULL	0	NULL	nuclear envelope 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These results point to a neuroprotective role for GM1 and its associated exchanger in the nucleus , based on regulation of Ca2 + flux between nucleoplasm and nuclear envelope .
	manualset3
179704	1	413895	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results propose a direct interaction between the calmodulin binding auto-inhibitory domain of the PM Ca ( 2 + ) - ATPase and the specific regions of the Na + , K ( + ) - ATPase alpha 1 subunit that are structurally homologous to the PM Ca ( 2 + ) - ATPase .
	manualset3
179705	2	413895	7	NULL	NULL	0	NULL	direct interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results propose a direct interaction between the calmodulin binding auto-inhibitory domain of the PM Ca ( 2 + ) - ATPase and the specific regions of the Na + , K ( + ) - ATPase alpha 1 subunit that are structurally homologous to the PM Ca ( 2 + ) - ATPase .
	manualset3
179706	3	413895	7	NULL	NULL	0	NULL	calmodulin binding auto-inhibitory domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results propose a direct interaction between the calmodulin binding auto-inhibitory domain of the PM Ca ( 2 + ) - ATPase and the specific regions of the Na + , K ( + ) - ATPase alpha 1 subunit that are structurally homologous to the PM Ca ( 2 + ) - ATPase .
	manualset3
179707	4	413895	7	NULL	NULL	0	NULL	PM Ca ( 2 + ) - ATPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results propose a direct interaction between the calmodulin binding auto-inhibitory domain of the PM Ca ( 2 + ) - ATPase and the specific regions of the Na + , K ( + ) - ATPase alpha 1 subunit that are structurally homologous to the PM Ca ( 2 + ) - ATPase .
	manualset3
179731	5	413895	7	NULL	NULL	0	NULL	specific regions	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results propose a direct interaction between the calmodulin binding auto-inhibitory domain of the PM Ca ( 2 + ) - ATPase and the specific regions of the Na + , K ( + ) - ATPase alpha 1 subunit that are structurally homologous to the PM Ca ( 2 + ) - ATPase .
	manualset3
179732	6	413895	7	NULL	NULL	0	NULL	Na + , K ( + ) - ATPase alpha 1 subunit	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results propose a direct interaction between the calmodulin binding auto-inhibitory domain of the PM Ca ( 2 + ) - ATPase and the specific regions of the Na + , K ( + ) - ATPase alpha 1 subunit that are structurally homologous to the PM Ca ( 2 + ) - ATPase .
	manualset3
179735	7	413895	7	NULL	NULL	0	NULL	 PM Ca ( 2 + ) - ATPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results propose a direct interaction between the calmodulin binding auto-inhibitory domain of the PM Ca ( 2 + ) - ATPase and the specific regions of the Na + , K ( + ) - ATPase alpha 1 subunit that are structurally homologous to the PM Ca ( 2 + ) - ATPase .
	manualset3
179736	1	413896	7	NULL	NULL	0	NULL	 results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide a further indication that group II pathways gives rise to the heteronymous late CPN-induced excitation .
	manualset3
179737	2	413896	7	NULL	NULL	NULL	NULL	 indication	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results provide a further indication that group II pathways gives rise to the heteronymous late CPN-induced excitation .
	manualset3
179738	3	413896	7	NULL	NULL	0	NULL	group II pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide a further indication that group II pathways gives rise to the heteronymous late CPN-induced excitation .
	manualset3
179739	4	413896	7	NULL	NULL	0	NULL	heteronymous late CPN-induced excitation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide a further indication that group II pathways gives rise to the heteronymous late CPN-induced excitation .
	manualset3
179740	1	413897	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide additional evidence for the discriminant validity of this particular battery of tests , and explicate further the skills and abilities measured in neuropsychological assessments of children referred for evaluation .
	manualset3
179741	2	413897	7	NULL	NULL	0	NULL	 evidence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide additional evidence for the discriminant validity of this particular battery of tests , and explicate further the skills and abilities measured in neuropsychological assessments of children referred for evaluation .
	manualset3
179742	3	413897	7	NULL	NULL	0	NULL	discriminant validity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide additional evidence for the discriminant validity of this particular battery of tests , and explicate further the skills and abilities measured in neuropsychological assessments of children referred for evaluation .
	manualset3
179743	4	413897	7	NULL	NULL	0	NULL	battery of tests 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide additional evidence for the discriminant validity of this particular battery of tests , and explicate further the skills and abilities measured in neuropsychological assessments of children referred for evaluation .
	manualset3
179744	5	413897	7	NULL	NULL	NULL	NULL	skills	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results provide additional evidence for the discriminant validity of this particular battery of tests , and explicate further the skills and abilities measured in neuropsychological assessments of children referred for evaluation .
	manualset3
179745	6	413897	7	NULL	NULL	0	NULL	abilities 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide additional evidence for the discriminant validity of this particular battery of tests , and explicate further the skills and abilities measured in neuropsychological assessments of children referred for evaluation .
	manualset3
179746	7	413897	7	NULL	NULL	0	NULL	 neuropsychological assessments	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide additional evidence for the discriminant validity of this particular battery of tests , and explicate further the skills and abilities measured in neuropsychological assessments of children referred for evaluation .
	manualset3
179747	8	413897	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide additional evidence for the discriminant validity of this particular battery of tests , and explicate further the skills and abilities measured in neuropsychological assessments of children referred for evaluation .
	manualset3
179748	9	413897	7	NULL	NULL	0	NULL	evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide additional evidence for the discriminant validity of this particular battery of tests , and explicate further the skills and abilities measured in neuropsychological assessments of children referred for evaluation .
	manualset3
179749	1	413898	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide evidence that in a folate-deficient rat model , both homocysteine and glycine are sensitive to dietary folic acid levels ; however , the observed hyperglycinemia does not appear to be related to a reduced flux through the hepatic GCS .
	manualset3
179750	2	413898	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide evidence that in a folate-deficient rat model , both homocysteine and glycine are sensitive to dietary folic acid levels ; however , the observed hyperglycinemia does not appear to be related to a reduced flux through the hepatic GCS .
	manualset3
179751	3	413898	7	NULL	NULL	0	NULL	 folate-deficient rat model	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide evidence that in a folate-deficient rat model , both homocysteine and glycine are sensitive to dietary folic acid levels ; however , the observed hyperglycinemia does not appear to be related to a reduced flux through the hepatic GCS .
	manualset3
179752	4	413898	7	NULL	NULL	0	NULL	homocysteine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide evidence that in a folate-deficient rat model , both homocysteine and glycine are sensitive to dietary folic acid levels ; however , the observed hyperglycinemia does not appear to be related to a reduced flux through the hepatic GCS .
	manualset3
179753	5	413898	7	NULL	NULL	0	NULL	glycine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide evidence that in a folate-deficient rat model , both homocysteine and glycine are sensitive to dietary folic acid levels ; however , the observed hyperglycinemia does not appear to be related to a reduced flux through the hepatic GCS .
	manualset3
179755	6	413898	7	NULL	NULL	0	NULL	dietary folic acid levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide evidence that in a folate-deficient rat model , both homocysteine and glycine are sensitive to dietary folic acid levels ; however , the observed hyperglycinemia does not appear to be related to a reduced flux through the hepatic GCS .
	manualset3
179758	7	413898	7	NULL	NULL	0	NULL	observed hyperglycinemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide evidence that in a folate-deficient rat model , both homocysteine and glycine are sensitive to dietary folic acid levels ; however , the observed hyperglycinemia does not appear to be related to a reduced flux through the hepatic GCS .
	manualset3
179759	8	413898	7	NULL	NULL	0	NULL	 reduced flux	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide evidence that in a folate-deficient rat model , both homocysteine and glycine are sensitive to dietary folic acid levels ; however , the observed hyperglycinemia does not appear to be related to a reduced flux through the hepatic GCS .
	manualset3
179770	9	413898	7	NULL	NULL	0	NULL	hepatic GCS	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide evidence that in a folate-deficient rat model , both homocysteine and glycine are sensitive to dietary folic acid levels ; however , the observed hyperglycinemia does not appear to be related to a reduced flux through the hepatic GCS .
	manualset3
179771	1	413899	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide further evidence for the functional importance of TPJ suppression and indicate that TPJ and DMN deactivation is especially critical during WM trace formation .
	manualset3
179772	2	413899	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide further evidence for the functional importance of TPJ suppression and indicate that TPJ and DMN deactivation is especially critical during WM trace formation .
	manualset3
179773	3	413899	7	NULL	NULL	0	NULL	functional importance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide further evidence for the functional importance of TPJ suppression and indicate that TPJ and DMN deactivation is especially critical during WM trace formation .
	manualset3
179774	4	413899	7	NULL	NULL	0	NULL	TPJ suppression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide further evidence for the functional importance of TPJ suppression and indicate that TPJ and DMN deactivation is especially critical during WM trace formation .
	manualset3
179775	5	413899	7	NULL	NULL	0	NULL	TPJ deactivation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide further evidence for the functional importance of TPJ suppression and indicate that TPJ and DMN deactivation is especially critical during WM trace formation .
	manualset3
179776	6	413899	7	NULL	NULL	0	NULL	DMN deactivation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide further evidence for the functional importance of TPJ suppression and indicate that TPJ and DMN deactivation is especially critical during WM trace formation .
	manualset3
179777	7	413899	7	NULL	NULL	0	NULL	WM trace formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide further evidence for the functional importance of TPJ suppression and indicate that TPJ and DMN deactivation is especially critical during WM trace formation .
	manualset3
179778	1	413900	7	NULL	NULL	0	NULL	 topical therapies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional topical therapies including benzoyl peroxide , clindamycin , retinoids , topical steroids , calcineurin inhibitors , and permethrin are not approved for the treatment of rosacea and play variable roles in the management of this condition .
	manualset3
179779	2	413900	7	NULL	NULL	NULL	NULL	benzoyl peroxide	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Additional topical therapies including benzoyl peroxide , clindamycin , retinoids , topical steroids , calcineurin inhibitors , and permethrin are not approved for the treatment of rosacea and play variable roles in the management of this condition .
	manualset3
179780	3	413900	7	NULL	NULL	NULL	NULL	clindamycin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Additional topical therapies including benzoyl peroxide , clindamycin , retinoids , topical steroids , calcineurin inhibitors , and permethrin are not approved for the treatment of rosacea and play variable roles in the management of this condition .
	manualset3
179781	4	413900	7	NULL	NULL	NULL	NULL	retinoids	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Additional topical therapies including benzoyl peroxide , clindamycin , retinoids , topical steroids , calcineurin inhibitors , and permethrin are not approved for the treatment of rosacea and play variable roles in the management of this condition .
	manualset3
179782	5	413900	7	NULL	NULL	NULL	NULL	topical steroids	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Additional topical therapies including benzoyl peroxide , clindamycin , retinoids , topical steroids , calcineurin inhibitors , and permethrin are not approved for the treatment of rosacea and play variable roles in the management of this condition .
	manualset3
179783	6	413900	7	NULL	NULL	NULL	NULL	calcineurin inhibitors 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Additional topical therapies including benzoyl peroxide , clindamycin , retinoids , topical steroids , calcineurin inhibitors , and permethrin are not approved for the treatment of rosacea and play variable roles in the management of this condition .
	manualset3
179784	7	413900	7	NULL	NULL	0	NULL	permethrin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional topical therapies including benzoyl peroxide , clindamycin , retinoids , topical steroids , calcineurin inhibitors , and permethrin are not approved for the treatment of rosacea and play variable roles in the management of this condition .
	manualset3
179785	8	413900	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional topical therapies including benzoyl peroxide , clindamycin , retinoids , topical steroids , calcineurin inhibitors , and permethrin are not approved for the treatment of rosacea and play variable roles in the management of this condition .
	manualset3
179786	9	413900	7	NULL	NULL	0	NULL	rosacea	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional topical therapies including benzoyl peroxide , clindamycin , retinoids , topical steroids , calcineurin inhibitors , and permethrin are not approved for the treatment of rosacea and play variable roles in the management of this condition .
	manualset3
179787	10	413900	7	NULL	NULL	0	NULL	roles	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional topical therapies including benzoyl peroxide , clindamycin , retinoids , topical steroids , calcineurin inhibitors , and permethrin are not approved for the treatment of rosacea and play variable roles in the management of this condition .
	manualset3
179788	11	413900	7	NULL	NULL	0	NULL	management 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional topical therapies including benzoyl peroxide , clindamycin , retinoids , topical steroids , calcineurin inhibitors , and permethrin are not approved for the treatment of rosacea and play variable roles in the management of this condition .
	manualset3
179789	12	413900	7	NULL	NULL	0	NULL	condition	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional topical therapies including benzoyl peroxide , clindamycin , retinoids , topical steroids , calcineurin inhibitors , and permethrin are not approved for the treatment of rosacea and play variable roles in the management of this condition .
	manualset3
179801	1	413901	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide in vivo evidence for an exceptionally stable lockdown mechanism to retain all loaded Mcm proteins on chromatin throughout prolonged cell cycles .
	manualset3
179804	2	413901	7	NULL	NULL	0	NULL	in vivo evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide in vivo evidence for an exceptionally stable lockdown mechanism to retain all loaded Mcm proteins on chromatin throughout prolonged cell cycles .
	manualset3
179811	3	413901	7	NULL	NULL	0	NULL	exceptionally stable lockdown mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide in vivo evidence for an exceptionally stable lockdown mechanism to retain all loaded Mcm proteins on chromatin throughout prolonged cell cycles .
	manualset3
179815	4	413901	7	NULL	NULL	0	NULL	Mcm proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide in vivo evidence for an exceptionally stable lockdown mechanism to retain all loaded Mcm proteins on chromatin throughout prolonged cell cycles .
	manualset3
179818	5	413901	7	NULL	NULL	0	NULL	chromatin 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide in vivo evidence for an exceptionally stable lockdown mechanism to retain all loaded Mcm proteins on chromatin throughout prolonged cell cycles .
	manualset3
179819	6	413901	7	NULL	NULL	0	NULL	cell cycles	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide in vivo evidence for an exceptionally stable lockdown mechanism to retain all loaded Mcm proteins on chromatin throughout prolonged cell cycles .
	manualset3
179823	1	413902	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide information for the development of knowledge-based intervention methods against this pathogen , as well as provide insight into potential mechanisms of cross-protection .
	manualset3
179825	2	413902	7	NULL	NULL	0	NULL	 information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide information for the development of knowledge-based intervention methods against this pathogen , as well as provide insight into potential mechanisms of cross-protection .
	manualset3
179826	3	413902	7	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide information for the development of knowledge-based intervention methods against this pathogen , as well as provide insight into potential mechanisms of cross-protection .
	manualset3
179827	4	413902	7	NULL	NULL	0	NULL	knowledge-based intervention methods	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide information for the development of knowledge-based intervention methods against this pathogen , as well as provide insight into potential mechanisms of cross-protection .
	manualset3
179828	5	413902	7	NULL	NULL	0	NULL	pathogen	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide information for the development of knowledge-based intervention methods against this pathogen , as well as provide insight into potential mechanisms of cross-protection .
	manualset3
179829	6	413902	7	NULL	NULL	0	NULL	potential mechanisms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide information for the development of knowledge-based intervention methods against this pathogen , as well as provide insight into potential mechanisms of cross-protection .
	manualset3
179830	7	413902	7	NULL	NULL	0	NULL	cross-protection 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide information for the development of knowledge-based intervention methods against this pathogen , as well as provide insight into potential mechanisms of cross-protection .
	manualset3
179858	1	413903	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide morphological evidence that a subset of the PR-IR neurons expressing SOM in the VL have long projections to the midbrain and suggest that the SOM system may modulate neural circuits involved in the regulation of steroid-influenced behaviors and neuroendocrine functions .
	manualset3
179860	2	413903	7	NULL	NULL	0	NULL	morphological evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide morphological evidence that a subset of the PR-IR neurons expressing SOM in the VL have long projections to the midbrain and suggest that the SOM system may modulate neural circuits involved in the regulation of steroid-influenced behaviors and neuroendocrine functions .
	manualset3
179861	3	413903	7	NULL	NULL	0	NULL	subset 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide morphological evidence that a subset of the PR-IR neurons expressing SOM in the VL have long projections to the midbrain and suggest that the SOM system may modulate neural circuits involved in the regulation of steroid-influenced behaviors and neuroendocrine functions .
	manualset3
179862	4	413903	7	NULL	NULL	0	NULL	PR-IR neurons 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide morphological evidence that a subset of the PR-IR neurons expressing SOM in the VL have long projections to the midbrain and suggest that the SOM system may modulate neural circuits involved in the regulation of steroid-influenced behaviors and neuroendocrine functions .
	manualset3
179863	5	413903	7	NULL	NULL	NULL	NULL	SOM	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results provide morphological evidence that a subset of the PR-IR neurons expressing SOM in the VL have long projections to the midbrain and suggest that the SOM system may modulate neural circuits involved in the regulation of steroid-influenced behaviors and neuroendocrine functions .
	manualset3
179864	6	413903	7	NULL	NULL	0	NULL	VL	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide morphological evidence that a subset of the PR-IR neurons expressing SOM in the VL have long projections to the midbrain and suggest that the SOM system may modulate neural circuits involved in the regulation of steroid-influenced behaviors and neuroendocrine functions .
	manualset3
179865	7	413903	7	NULL	NULL	NULL	NULL	long projections 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results provide morphological evidence that a subset of the PR-IR neurons expressing SOM in the VL have long projections to the midbrain and suggest that the SOM system may modulate neural circuits involved in the regulation of steroid-influenced behaviors and neuroendocrine functions .
	manualset3
179866	8	413903	7	NULL	NULL	0	NULL	midbrain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide morphological evidence that a subset of the PR-IR neurons expressing SOM in the VL have long projections to the midbrain and suggest that the SOM system may modulate neural circuits involved in the regulation of steroid-influenced behaviors and neuroendocrine functions .
	manualset3
179867	9	413903	7	NULL	NULL	0	NULL	SOM system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide morphological evidence that a subset of the PR-IR neurons expressing SOM in the VL have long projections to the midbrain and suggest that the SOM system may modulate neural circuits involved in the regulation of steroid-influenced behaviors and neuroendocrine functions .
	manualset3
179868	10	413903	7	NULL	NULL	0	NULL	neural circuits	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide morphological evidence that a subset of the PR-IR neurons expressing SOM in the VL have long projections to the midbrain and suggest that the SOM system may modulate neural circuits involved in the regulation of steroid-influenced behaviors and neuroendocrine functions .
	manualset3
179869	11	413903	7	NULL	NULL	0	NULL	 regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide morphological evidence that a subset of the PR-IR neurons expressing SOM in the VL have long projections to the midbrain and suggest that the SOM system may modulate neural circuits involved in the regulation of steroid-influenced behaviors and neuroendocrine functions .
	manualset3
179870	12	413903	7	NULL	NULL	0	NULL	steroid-influenced behaviors	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide morphological evidence that a subset of the PR-IR neurons expressing SOM in the VL have long projections to the midbrain and suggest that the SOM system may modulate neural circuits involved in the regulation of steroid-influenced behaviors and neuroendocrine functions .
	manualset3
179873	13	413903	7	NULL	NULL	0	NULL	neuroendocrine functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide morphological evidence that a subset of the PR-IR neurons expressing SOM in the VL have long projections to the midbrain and suggest that the SOM system may modulate neural circuits involved in the regulation of steroid-influenced behaviors and neuroendocrine functions .
	manualset3
179942	1	413904	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results raise the question whether AAV persists better in eyes than adenovirus or that a possible association with conjunctivitis might be present .
	manualset3
179943	2	413904	7	NULL	NULL	0	NULL	 AAV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results raise the question whether AAV persists better in eyes than adenovirus or that a possible association with conjunctivitis might be present .
	manualset3
179944	3	413904	7	NULL	NULL	0	NULL	eyes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results raise the question whether AAV persists better in eyes than adenovirus or that a possible association with conjunctivitis might be present .
	manualset3
179945	4	413904	7	NULL	NULL	0	NULL	adenovirus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results raise the question whether AAV persists better in eyes than adenovirus or that a possible association with conjunctivitis might be present .
	manualset3
179946	5	413904	7	NULL	NULL	NULL	NULL	association	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results raise the question whether AAV persists better in eyes than adenovirus or that a possible association with conjunctivitis might be present .
	manualset3
179947	6	413904	7	NULL	NULL	NULL	NULL	conjunctivitis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results raise the question whether AAV persists better in eyes than adenovirus or that a possible association with conjunctivitis might be present .
	manualset3
179948	7	413904	7	NULL	NULL	0	NULL	 question	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results raise the question whether AAV persists better in eyes than adenovirus or that a possible association with conjunctivitis might be present .
	manualset3
179949	1	413905	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results reemphasize the inadequacy of screening only those patients with traditional risk factors for gestational diabetes and demonstrate the feasibility of implementing a program of universal glucose screening among a large obstetric population .
	manualset3
179950	2	413905	7	NULL	NULL	0	NULL	 inadequacy of screening	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results reemphasize the inadequacy of screening only those patients with traditional risk factors for gestational diabetes and demonstrate the feasibility of implementing a program of universal glucose screening among a large obstetric population .
	manualset3
179951	3	413905	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results reemphasize the inadequacy of screening only those patients with traditional risk factors for gestational diabetes and demonstrate the feasibility of implementing a program of universal glucose screening among a large obstetric population .
	manualset3
179952	4	413905	7	NULL	NULL	0	NULL	traditional risk factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results reemphasize the inadequacy of screening only those patients with traditional risk factors for gestational diabetes and demonstrate the feasibility of implementing a program of universal glucose screening among a large obstetric population .
	manualset3
179953	5	413905	7	NULL	NULL	0	NULL	gestational diabetes 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results reemphasize the inadequacy of screening only those patients with traditional risk factors for gestational diabetes and demonstrate the feasibility of implementing a program of universal glucose screening among a large obstetric population .
	manualset3
179954	6	413905	7	NULL	NULL	0	NULL	feasibility	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results reemphasize the inadequacy of screening only those patients with traditional risk factors for gestational diabetes and demonstrate the feasibility of implementing a program of universal glucose screening among a large obstetric population .
	manualset3
179955	7	413905	7	NULL	NULL	0	NULL	implementing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results reemphasize the inadequacy of screening only those patients with traditional risk factors for gestational diabetes and demonstrate the feasibility of implementing a program of universal glucose screening among a large obstetric population .
	manualset3
179956	8	413905	7	NULL	NULL	0	NULL	program 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	These results reemphasize the inadequacy of screening only those patients with traditional risk factors for gestational diabetes and demonstrate the feasibility of implementing a program of universal glucose screening among a large obstetric population .
	manualset3
179957	9	413905	7	NULL	NULL	0	NULL	universal glucose screening	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results reemphasize the inadequacy of screening only those patients with traditional risk factors for gestational diabetes and demonstrate the feasibility of implementing a program of universal glucose screening among a large obstetric population .
	manualset3
179958	10	413905	7	NULL	NULL	0	NULL	obstetric population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results reemphasize the inadequacy of screening only those patients with traditional risk factors for gestational diabetes and demonstrate the feasibility of implementing a program of universal glucose screening among a large obstetric population .
	manualset3
179959	1	413906	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results reveal that target detection is not a single cognitive event , but rather a process of progressive target selectivity that involves large-scale rapid parallel and serial processing in sensory , cognitive , and motor structures to support goal-directed human behavior .
	manualset3
179960	2	413906	7	NULL	NULL	NULL	NULL	target detection 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results reveal that target detection is not a single cognitive event , but rather a process of progressive target selectivity that involves large-scale rapid parallel and serial processing in sensory , cognitive , and motor structures to support goal-directed human behavior .
	manualset3
179961	3	413906	7	NULL	NULL	0	NULL	single cognitive event	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results reveal that target detection is not a single cognitive event , but rather a process of progressive target selectivity that involves large-scale rapid parallel and serial processing in sensory , cognitive , and motor structures to support goal-directed human behavior .
	manualset3
179962	4	413906	7	NULL	NULL	0	NULL	process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results reveal that target detection is not a single cognitive event , but rather a process of progressive target selectivity that involves large-scale rapid parallel and serial processing in sensory , cognitive , and motor structures to support goal-directed human behavior .
	manualset3
179963	5	413906	7	NULL	NULL	0	NULL	progressive target selectivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results reveal that target detection is not a single cognitive event , but rather a process of progressive target selectivity that involves large-scale rapid parallel and serial processing in sensory , cognitive , and motor structures to support goal-directed human behavior .
	manualset3
179964	6	413906	7	NULL	NULL	0	NULL	large-scale rapid parallel processing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results reveal that target detection is not a single cognitive event , but rather a process of progressive target selectivity that involves large-scale rapid parallel and serial processing in sensory , cognitive , and motor structures to support goal-directed human behavior .
	manualset3
179965	7	413906	7	NULL	NULL	0	NULL	serial processing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results reveal that target detection is not a single cognitive event , but rather a process of progressive target selectivity that involves large-scale rapid parallel and serial processing in sensory , cognitive , and motor structures to support goal-directed human behavior .
	manualset3
179966	8	413906	7	NULL	NULL	0	NULL	sensory structures	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results reveal that target detection is not a single cognitive event , but rather a process of progressive target selectivity that involves large-scale rapid parallel and serial processing in sensory , cognitive , and motor structures to support goal-directed human behavior .
	manualset3
179967	9	413906	7	NULL	NULL	0	NULL	cognitive structures	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results reveal that target detection is not a single cognitive event , but rather a process of progressive target selectivity that involves large-scale rapid parallel and serial processing in sensory , cognitive , and motor structures to support goal-directed human behavior .
	manualset3
179968	10	413906	7	NULL	NULL	0	NULL	motor structures 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results reveal that target detection is not a single cognitive event , but rather a process of progressive target selectivity that involves large-scale rapid parallel and serial processing in sensory , cognitive , and motor structures to support goal-directed human behavior .
	manualset3
179969	11	413906	7	NULL	NULL	0	NULL	goal-directed human behavior	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results reveal that target detection is not a single cognitive event , but rather a process of progressive target selectivity that involves large-scale rapid parallel and serial processing in sensory , cognitive , and motor structures to support goal-directed human behavior .
	manualset3
179970	1	413907	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results revealed that most microorganisms belonged to the genus Bacillus and presented alcohol dehydrogenase , monooxygenase , epoxide hydrolase , esterase , and lipase activities .
	manualset3
179971	2	413907	7	NULL	NULL	0	NULL	microorganisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results revealed that most microorganisms belonged to the genus Bacillus and presented alcohol dehydrogenase , monooxygenase , epoxide hydrolase , esterase , and lipase activities .
	manualset3
179972	3	413907	7	NULL	NULL	0	NULL	genus Bacillus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results revealed that most microorganisms belonged to the genus Bacillus and presented alcohol dehydrogenase , monooxygenase , epoxide hydrolase , esterase , and lipase activities .
	manualset3
179973	4	413907	7	NULL	NULL	NULL	NULL	alcohol dehydrogenase activities	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results revealed that most microorganisms belonged to the genus Bacillus and presented alcohol dehydrogenase , monooxygenase , epoxide hydrolase , esterase , and lipase activities .
	manualset3
179974	5	413907	7	NULL	NULL	NULL	NULL	monooxygenase activities	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results revealed that most microorganisms belonged to the genus Bacillus and presented alcohol dehydrogenase , monooxygenase , epoxide hydrolase , esterase , and lipase activities .
	manualset3
179975	6	413907	7	NULL	NULL	NULL	NULL	epoxide hydrolase activities	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results revealed that most microorganisms belonged to the genus Bacillus and presented alcohol dehydrogenase , monooxygenase , epoxide hydrolase , esterase , and lipase activities .
	manualset3
179976	7	413907	7	NULL	NULL	0	NULL	esterase activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results revealed that most microorganisms belonged to the genus Bacillus and presented alcohol dehydrogenase , monooxygenase , epoxide hydrolase , esterase , and lipase activities .
	manualset3
179977	8	413907	7	NULL	NULL	0	NULL	lipase activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results revealed that most microorganisms belonged to the genus Bacillus and presented alcohol dehydrogenase , monooxygenase , epoxide hydrolase , esterase , and lipase activities .
	manualset3
179978	1	413908	7	NULL	NULL	0	NULL	 results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that COS-7 cells express a K + channel with unique properties that must be considered when using these cells as transfection system .
	manualset3
179979	2	413908	7	NULL	NULL	0	NULL	COS-7 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that COS-7 cells express a K + channel with unique properties that must be considered when using these cells as transfection system .
	manualset3
179980	3	413908	7	NULL	NULL	0	NULL	K + channel	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that COS-7 cells express a K + channel with unique properties that must be considered when using these cells as transfection system .
	manualset3
179981	4	413908	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that COS-7 cells express a K + channel with unique properties that must be considered when using these cells as transfection system .
	manualset3
179982	5	413908	7	NULL	NULL	0	NULL	transfection system	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that COS-7 cells express a K + channel with unique properties that must be considered when using these cells as transfection system .
	manualset3
179983	1	413909	7	NULL	NULL	0	NULL	Comparative study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative study of plasma levels of 8-methoxypsoralen .
	manualset3
179984	2	413909	7	NULL	NULL	0	NULL	plasma levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative study of plasma levels of 8-methoxypsoralen .
	manualset3
179985	3	413909	7	NULL	NULL	0	NULL	8-methoxypsoralen	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative study of plasma levels of 8-methoxypsoralen .
	manualset3
179986	1	413910	7	NULL	NULL	0	NULL	 results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that TESPtBC may be a viable precursor for applications in acid-base cooperative CO ( 2 ) conversion catalysts , and that variation in the local amine surface density and the chemistry of the underlying support may account for some of the large variability in reported CO ( 2 ) capacities of supported amine materials in literature .
	manualset3
179987	2	413910	7	NULL	NULL	0	NULL	TESPtBC	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that TESPtBC may be a viable precursor for applications in acid-base cooperative CO ( 2 ) conversion catalysts , and that variation in the local amine surface density and the chemistry of the underlying support may account for some of the large variability in reported CO ( 2 ) capacities of supported amine materials in literature .
	manualset3
179988	3	413910	7	NULL	NULL	0	NULL	viable precursor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that TESPtBC may be a viable precursor for applications in acid-base cooperative CO ( 2 ) conversion catalysts , and that variation in the local amine surface density and the chemistry of the underlying support may account for some of the large variability in reported CO ( 2 ) capacities of supported amine materials in literature .
	manualset3
179989	4	413910	7	NULL	NULL	NULL	NULL	applications	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results show that TESPtBC may be a viable precursor for applications in acid-base cooperative CO ( 2 ) conversion catalysts , and that variation in the local amine surface density and the chemistry of the underlying support may account for some of the large variability in reported CO ( 2 ) capacities of supported amine materials in literature .
	manualset3
179990	5	413910	7	NULL	NULL	0	NULL	acid-base cooperative CO ( 2 ) conversion catalysts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that TESPtBC may be a viable precursor for applications in acid-base cooperative CO ( 2 ) conversion catalysts , and that variation in the local amine surface density and the chemistry of the underlying support may account for some of the large variability in reported CO ( 2 ) capacities of supported amine materials in literature .
	manualset3
179991	6	413910	7	NULL	NULL	0	NULL	variation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that TESPtBC may be a viable precursor for applications in acid-base cooperative CO ( 2 ) conversion catalysts , and that variation in the local amine surface density and the chemistry of the underlying support may account for some of the large variability in reported CO ( 2 ) capacities of supported amine materials in literature .
	manualset3
179992	7	413910	7	NULL	NULL	0	NULL	local amine surface density	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that TESPtBC may be a viable precursor for applications in acid-base cooperative CO ( 2 ) conversion catalysts , and that variation in the local amine surface density and the chemistry of the underlying support may account for some of the large variability in reported CO ( 2 ) capacities of supported amine materials in literature .
	manualset3
179993	8	413910	7	NULL	NULL	0	NULL	 chemistry	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that TESPtBC may be a viable precursor for applications in acid-base cooperative CO ( 2 ) conversion catalysts , and that variation in the local amine surface density and the chemistry of the underlying support may account for some of the large variability in reported CO ( 2 ) capacities of supported amine materials in literature .
	manualset3
179994	9	413910	7	NULL	NULL	0	NULL	underlying support	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that TESPtBC may be a viable precursor for applications in acid-base cooperative CO ( 2 ) conversion catalysts , and that variation in the local amine surface density and the chemistry of the underlying support may account for some of the large variability in reported CO ( 2 ) capacities of supported amine materials in literature .
	manualset3
179995	10	413910	7	NULL	NULL	0	NULL	large variability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that TESPtBC may be a viable precursor for applications in acid-base cooperative CO ( 2 ) conversion catalysts , and that variation in the local amine surface density and the chemistry of the underlying support may account for some of the large variability in reported CO ( 2 ) capacities of supported amine materials in literature .
	manualset3
179996	11	413910	7	NULL	NULL	0	NULL	CO ( 2 ) capacities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that TESPtBC may be a viable precursor for applications in acid-base cooperative CO ( 2 ) conversion catalysts , and that variation in the local amine surface density and the chemistry of the underlying support may account for some of the large variability in reported CO ( 2 ) capacities of supported amine materials in literature .
	manualset3
179997	12	413910	7	NULL	NULL	0	NULL	amine materials	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that TESPtBC may be a viable precursor for applications in acid-base cooperative CO ( 2 ) conversion catalysts , and that variation in the local amine surface density and the chemistry of the underlying support may account for some of the large variability in reported CO ( 2 ) capacities of supported amine materials in literature .
	manualset3
179998	13	413910	7	NULL	NULL	0	NULL	literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that TESPtBC may be a viable precursor for applications in acid-base cooperative CO ( 2 ) conversion catalysts , and that variation in the local amine surface density and the chemistry of the underlying support may account for some of the large variability in reported CO ( 2 ) capacities of supported amine materials in literature .
	manualset3
179999	1	413911	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that a virion association motif for Vpr is located within residues 1 to 46 of p6 .
	manualset3
180000	2	413911	7	NULL	NULL	0	NULL	virion association motif	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that a virion association motif for Vpr is located within residues 1 to 46 of p6 .
	manualset3
180009	3	413911	7	NULL	NULL	0	NULL	Vpr	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that a virion association motif for Vpr is located within residues 1 to 46 of p6 .
	manualset3
180010	4	413911	7	NULL	NULL	0	NULL	residues 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that a virion association motif for Vpr is located within residues 1 to 46 of p6 .
	manualset3
180011	5	413911	7	NULL	NULL	0	NULL	1 to 46	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that a virion association motif for Vpr is located within residues 1 to 46 of p6 .
	manualset3
180012	6	413911	7	NULL	NULL	0	NULL	p6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that a virion association motif for Vpr is located within residues 1 to 46 of p6 .
	manualset3
180013	1	413912	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that actin can migrate in agarose gels in the F form and that it is oriented during the electrophoresis .
	manualset3
180014	2	413912	7	NULL	NULL	0	NULL	actin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that actin can migrate in agarose gels in the F form and that it is oriented during the electrophoresis .
	manualset3
180016	3	413912	7	NULL	NULL	0	NULL	agarose gels	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that actin can migrate in agarose gels in the F form and that it is oriented during the electrophoresis .
	manualset3
180018	4	413912	7	NULL	NULL	0	NULL	F form	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that actin can migrate in agarose gels in the F form and that it is oriented during the electrophoresis .
	manualset3
180021	5	413912	7	NULL	NULL	0	NULL	electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that actin can migrate in agarose gels in the F form and that it is oriented during the electrophoresis .
	manualset3
180022	1	413913	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that discriminative stimulus effects of nicotine are not fixed properties of the drug , but can be influenced by training conditions , and that effects associated with this discrimination may differ between men and women .
	manualset3
180023	2	413913	7	NULL	NULL	0	NULL	discriminative stimulus effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that discriminative stimulus effects of nicotine are not fixed properties of the drug , but can be influenced by training conditions , and that effects associated with this discrimination may differ between men and women .
	manualset3
180024	3	413913	7	NULL	NULL	0	NULL	nicotine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that discriminative stimulus effects of nicotine are not fixed properties of the drug , but can be influenced by training conditions , and that effects associated with this discrimination may differ between men and women .
	manualset3
180025	4	413913	7	NULL	NULL	0	NULL	drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that discriminative stimulus effects of nicotine are not fixed properties of the drug , but can be influenced by training conditions , and that effects associated with this discrimination may differ between men and women .
	manualset3
180028	5	413913	7	NULL	NULL	0	NULL	training conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that discriminative stimulus effects of nicotine are not fixed properties of the drug , but can be influenced by training conditions , and that effects associated with this discrimination may differ between men and women .
	manualset3
180029	6	413913	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that discriminative stimulus effects of nicotine are not fixed properties of the drug , but can be influenced by training conditions , and that effects associated with this discrimination may differ between men and women .
	manualset3
180030	7	413913	7	NULL	NULL	0	NULL	discrimination	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that discriminative stimulus effects of nicotine are not fixed properties of the drug , but can be influenced by training conditions , and that effects associated with this discrimination may differ between men and women .
	manualset3
180031	8	413913	7	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that discriminative stimulus effects of nicotine are not fixed properties of the drug , but can be influenced by training conditions , and that effects associated with this discrimination may differ between men and women .
	manualset3
180032	9	413913	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that discriminative stimulus effects of nicotine are not fixed properties of the drug , but can be influenced by training conditions , and that effects associated with this discrimination may differ between men and women .
	manualset3
180034	10	413913	7	NULL	NULL	0	NULL	fixed properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that discriminative stimulus effects of nicotine are not fixed properties of the drug , but can be influenced by training conditions , and that effects associated with this discrimination may differ between men and women .
	manualset3
180038	1	413914	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that troglitazone and BRL 49653 have a specific , post-translational inhibitory effect on lipoprotein lipase in adipocytes , yet they promote lipid accumulation and differentiation in preadipocytes .
	manualset3
180041	2	413914	7	NULL	NULL	0	NULL	troglitazone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that troglitazone and BRL 49653 have a specific , post-translational inhibitory effect on lipoprotein lipase in adipocytes , yet they promote lipid accumulation and differentiation in preadipocytes .
	manualset3
180042	3	413914	7	NULL	NULL	0	NULL	BRL 49653	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that troglitazone and BRL 49653 have a specific , post-translational inhibitory effect on lipoprotein lipase in adipocytes , yet they promote lipid accumulation and differentiation in preadipocytes .
	manualset3
180043	4	413914	7	NULL	NULL	0	NULL	post-translational inhibitory effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that troglitazone and BRL 49653 have a specific , post-translational inhibitory effect on lipoprotein lipase in adipocytes , yet they promote lipid accumulation and differentiation in preadipocytes .
	manualset3
180044	5	413914	7	NULL	NULL	0	NULL	lipoprotein lipase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that troglitazone and BRL 49653 have a specific , post-translational inhibitory effect on lipoprotein lipase in adipocytes , yet they promote lipid accumulation and differentiation in preadipocytes .
	manualset3
180045	6	413914	7	NULL	NULL	0	NULL	adipocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that troglitazone and BRL 49653 have a specific , post-translational inhibitory effect on lipoprotein lipase in adipocytes , yet they promote lipid accumulation and differentiation in preadipocytes .
	manualset3
180048	7	413914	7	NULL	NULL	0	NULL	lipid accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that troglitazone and BRL 49653 have a specific , post-translational inhibitory effect on lipoprotein lipase in adipocytes , yet they promote lipid accumulation and differentiation in preadipocytes .
	manualset3
180049	8	413914	7	NULL	NULL	NULL	NULL	lipid differentiation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results show that troglitazone and BRL 49653 have a specific , post-translational inhibitory effect on lipoprotein lipase in adipocytes , yet they promote lipid accumulation and differentiation in preadipocytes .
	manualset3
180050	9	413914	7	NULL	NULL	0	NULL	preadipocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show that troglitazone and BRL 49653 have a specific , post-translational inhibitory effect on lipoprotein lipase in adipocytes , yet they promote lipid accumulation and differentiation in preadipocytes .
	manualset3
180088	1	413915	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results showed that dynamic properties of Con A receptor are apparently different which were regulated by the cell cycle .
	manualset3
180089	2	413915	7	NULL	NULL	0	NULL	dynamic properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results showed that dynamic properties of Con A receptor are apparently different which were regulated by the cell cycle .
	manualset3
180090	3	413915	7	NULL	NULL	0	NULL	Con A receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results showed that dynamic properties of Con A receptor are apparently different which were regulated by the cell cycle .
	manualset3
180091	4	413915	7	NULL	NULL	0	NULL	 cell cycle	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results showed that dynamic properties of Con A receptor are apparently different which were regulated by the cell cycle .
	manualset3
180092	1	413916	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results showed that phloretin and phloridzin could inhibit the modification of the arginine residue by MGO and that phloretin could directly participate in the reaction between the thiol group and MGO .
	manualset3
180093	2	413916	7	NULL	NULL	0	NULL	phloretin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results showed that phloretin and phloridzin could inhibit the modification of the arginine residue by MGO and that phloretin could directly participate in the reaction between the thiol group and MGO .
	manualset3
180094	3	413916	7	NULL	NULL	0	NULL	phloridzin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results showed that phloretin and phloridzin could inhibit the modification of the arginine residue by MGO and that phloretin could directly participate in the reaction between the thiol group and MGO .
	manualset3
180096	4	413916	7	NULL	NULL	0	NULL	modification	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results showed that phloretin and phloridzin could inhibit the modification of the arginine residue by MGO and that phloretin could directly participate in the reaction between the thiol group and MGO .
	manualset3
180097	5	413916	7	NULL	NULL	0	NULL	arginine residue 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These results showed that phloretin and phloridzin could inhibit the modification of the arginine residue by MGO and that phloretin could directly participate in the reaction between the thiol group and MGO .
	manualset3
180098	6	413916	7	NULL	NULL	0	NULL	MGO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results showed that phloretin and phloridzin could inhibit the modification of the arginine residue by MGO and that phloretin could directly participate in the reaction between the thiol group and MGO .
	manualset3
180099	7	413916	7	NULL	NULL	0	NULL	phloretin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results showed that phloretin and phloridzin could inhibit the modification of the arginine residue by MGO and that phloretin could directly participate in the reaction between the thiol group and MGO .
	manualset3
180100	8	413916	7	NULL	NULL	0	NULL	reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results showed that phloretin and phloridzin could inhibit the modification of the arginine residue by MGO and that phloretin could directly participate in the reaction between the thiol group and MGO .
	manualset3
180101	9	413916	7	NULL	NULL	0	NULL	thiol group	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results showed that phloretin and phloridzin could inhibit the modification of the arginine residue by MGO and that phloretin could directly participate in the reaction between the thiol group and MGO .
	manualset3
180102	10	413916	7	NULL	NULL	0	NULL	MGO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results showed that phloretin and phloridzin could inhibit the modification of the arginine residue by MGO and that phloretin could directly participate in the reaction between the thiol group and MGO .
	manualset3
180103	1	413917	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results stress the need to develop universal formulae for estimating body water compartments which would include race and pathology as independent parameters , in addition to BIA and anthropometric variables .
	manualset3
180104	2	413917	7	NULL	NULL	0	NULL	universal formulae	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These results stress the need to develop universal formulae for estimating body water compartments which would include race and pathology as independent parameters , in addition to BIA and anthropometric variables .
	manualset3
180105	3	413917	7	NULL	NULL	0	NULL	body water compartments	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results stress the need to develop universal formulae for estimating body water compartments which would include race and pathology as independent parameters , in addition to BIA and anthropometric variables .
	manualset3
180106	4	413917	7	NULL	NULL	0	NULL	race	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results stress the need to develop universal formulae for estimating body water compartments which would include race and pathology as independent parameters , in addition to BIA and anthropometric variables .
	manualset3
180107	5	413917	7	NULL	NULL	0	NULL	pathology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results stress the need to develop universal formulae for estimating body water compartments which would include race and pathology as independent parameters , in addition to BIA and anthropometric variables .
	manualset3
180108	6	413917	7	NULL	NULL	0	NULL	independent parameters	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results stress the need to develop universal formulae for estimating body water compartments which would include race and pathology as independent parameters , in addition to BIA and anthropometric variables .
	manualset3
180109	7	413917	7	NULL	NULL	0	NULL	BIA variable	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These results stress the need to develop universal formulae for estimating body water compartments which would include race and pathology as independent parameters , in addition to BIA and anthropometric variables .
	manualset3
180110	8	413917	7	NULL	NULL	0	NULL	anthropometric variables	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These results stress the need to develop universal formulae for estimating body water compartments which would include race and pathology as independent parameters , in addition to BIA and anthropometric variables .
	manualset3
180162	1	413918	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results strongly suggest that LPS induces the release of IL-12 , that IL-12 induces the production of IFN-gamma , and that IFN-gamma is the cytokine that primes macrophages and other cell types .
	manualset3
180163	2	413918	7	NULL	NULL	0	NULL	LPS	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results strongly suggest that LPS induces the release of IL-12 , that IL-12 induces the production of IFN-gamma , and that IFN-gamma is the cytokine that primes macrophages and other cell types .
	manualset3
180164	3	413918	7	NULL	NULL	0	NULL	release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results strongly suggest that LPS induces the release of IL-12 , that IL-12 induces the production of IFN-gamma , and that IFN-gamma is the cytokine that primes macrophages and other cell types .
	manualset3
180165	4	413918	7	NULL	NULL	NULL	NULL	IL-12	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results strongly suggest that LPS induces the release of IL-12 , that IL-12 induces the production of IFN-gamma , and that IFN-gamma is the cytokine that primes macrophages and other cell types .
	manualset3
180166	5	413918	7	NULL	NULL	0	NULL	IL-12	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results strongly suggest that LPS induces the release of IL-12 , that IL-12 induces the production of IFN-gamma , and that IFN-gamma is the cytokine that primes macrophages and other cell types .
	manualset3
180167	6	413918	7	NULL	NULL	0	NULL	production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results strongly suggest that LPS induces the release of IL-12 , that IL-12 induces the production of IFN-gamma , and that IFN-gamma is the cytokine that primes macrophages and other cell types .
	manualset3
180168	7	413918	7	NULL	NULL	0	NULL	IFN-gamma	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results strongly suggest that LPS induces the release of IL-12 , that IL-12 induces the production of IFN-gamma , and that IFN-gamma is the cytokine that primes macrophages and other cell types .
	manualset3
180169	8	413918	7	NULL	NULL	0	NULL	IFN-gamma	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results strongly suggest that LPS induces the release of IL-12 , that IL-12 induces the production of IFN-gamma , and that IFN-gamma is the cytokine that primes macrophages and other cell types .
	manualset3
180170	9	413918	7	NULL	NULL	0	NULL	cytokine	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results strongly suggest that LPS induces the release of IL-12 , that IL-12 induces the production of IFN-gamma , and that IFN-gamma is the cytokine that primes macrophages and other cell types .
	manualset3
180171	10	413918	7	NULL	NULL	0	NULL	macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results strongly suggest that LPS induces the release of IL-12 , that IL-12 induces the production of IFN-gamma , and that IFN-gamma is the cytokine that primes macrophages and other cell types .
	manualset3
180172	11	413918	7	NULL	NULL	0	NULL	cell types	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results strongly suggest that LPS induces the release of IL-12 , that IL-12 induces the production of IFN-gamma , and that IFN-gamma is the cytokine that primes macrophages and other cell types .
	manualset3
180173	1	413919	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results strongly suggest that all of the three post-fertilization events , cessation of sperm attraction , expression of surface adhesion , and progression of cell cycle , lie downstream of MAP kinase dephosphorylation that is triggered by a Ca2 + increase .
	manualset3
180174	2	413919	7	NULL	NULL	NULL	NULL	three post-fertilization events 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results strongly suggest that all of the three post-fertilization events , cessation of sperm attraction , expression of surface adhesion , and progression of cell cycle , lie downstream of MAP kinase dephosphorylation that is triggered by a Ca2 + increase .
	manualset3
180175	3	413919	7	NULL	NULL	NULL	NULL	cessation of sperm attraction	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results strongly suggest that all of the three post-fertilization events , cessation of sperm attraction , expression of surface adhesion , and progression of cell cycle , lie downstream of MAP kinase dephosphorylation that is triggered by a Ca2 + increase .
	manualset3
180177	5	413919	7	NULL	NULL	NULL	NULL	expression of surface adhesion	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results strongly suggest that all of the three post-fertilization events , cessation of sperm attraction , expression of surface adhesion , and progression of cell cycle , lie downstream of MAP kinase dephosphorylation that is triggered by a Ca2 + increase .
	manualset3
180179	7	413919	7	NULL	NULL	NULL	NULL	progression of cell cycle	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results strongly suggest that all of the three post-fertilization events , cessation of sperm attraction , expression of surface adhesion , and progression of cell cycle , lie downstream of MAP kinase dephosphorylation that is triggered by a Ca2 + increase .
	manualset3
180181	9	413919	7	NULL	NULL	0	NULL	downstream	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results strongly suggest that all of the three post-fertilization events , cessation of sperm attraction , expression of surface adhesion , and progression of cell cycle , lie downstream of MAP kinase dephosphorylation that is triggered by a Ca2 + increase .
	manualset3
180182	10	413919	7	NULL	NULL	0	NULL	MAP kinase dephosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results strongly suggest that all of the three post-fertilization events , cessation of sperm attraction , expression of surface adhesion , and progression of cell cycle , lie downstream of MAP kinase dephosphorylation that is triggered by a Ca2 + increase .
	manualset3
180183	11	413919	7	NULL	NULL	0	NULL	Ca2 + increase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results strongly suggest that all of the three post-fertilization events , cessation of sperm attraction , expression of surface adhesion , and progression of cell cycle , lie downstream of MAP kinase dephosphorylation that is triggered by a Ca2 + increase .
	manualset3
180184	1	413920	7	NULL	NULL	0	NULL	2 different holding periods	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , 2 different holding periods for small crates were compared to determine whether holding time influences C. perfringens recovery before and after cleaning .
	manualset3
180185	2	413920	7	NULL	NULL	0	NULL	small crates	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , 2 different holding periods for small crates were compared to determine whether holding time influences C. perfringens recovery before and after cleaning .
	manualset3
180186	3	413920	7	NULL	NULL	0	NULL	C. perfringens recovery	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , 2 different holding periods for small crates were compared to determine whether holding time influences C. perfringens recovery before and after cleaning .
	manualset3
180187	4	413920	7	NULL	NULL	0	NULL	cleaning	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , 2 different holding periods for small crates were compared to determine whether holding time influences C. perfringens recovery before and after cleaning .
	manualset3
180188	5	413920	7	NULL	NULL	0	NULL	holding time	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , 2 different holding periods for small crates were compared to determine whether holding time influences C. perfringens recovery before and after cleaning .
	manualset3
180189	1	413921	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results substantiate the conclusion that the involvement of the o-quinone / QM pathway in catechol toxicity depends on a combination between the rate of enzymatic formation of the o-quinone , the rate of isomerization to the more electrophilic QM , and the chemical reactivity of the quinoids .
	manualset3
180190	2	413921	7	NULL	NULL	0	NULL	conclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results substantiate the conclusion that the involvement of the o-quinone / QM pathway in catechol toxicity depends on a combination between the rate of enzymatic formation of the o-quinone , the rate of isomerization to the more electrophilic QM , and the chemical reactivity of the quinoids .
	manualset3
180191	3	413921	7	NULL	NULL	0	NULL	 involvement	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results substantiate the conclusion that the involvement of the o-quinone / QM pathway in catechol toxicity depends on a combination between the rate of enzymatic formation of the o-quinone , the rate of isomerization to the more electrophilic QM , and the chemical reactivity of the quinoids .
	manualset3
180192	4	413921	7	NULL	NULL	0	NULL	o-quinone / QM pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results substantiate the conclusion that the involvement of the o-quinone / QM pathway in catechol toxicity depends on a combination between the rate of enzymatic formation of the o-quinone , the rate of isomerization to the more electrophilic QM , and the chemical reactivity of the quinoids .
	manualset3
180193	5	413921	7	NULL	NULL	0	NULL	catechol toxicity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results substantiate the conclusion that the involvement of the o-quinone / QM pathway in catechol toxicity depends on a combination between the rate of enzymatic formation of the o-quinone , the rate of isomerization to the more electrophilic QM , and the chemical reactivity of the quinoids .
	manualset3
180194	6	413921	7	NULL	NULL	0	NULL	combination	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results substantiate the conclusion that the involvement of the o-quinone / QM pathway in catechol toxicity depends on a combination between the rate of enzymatic formation of the o-quinone , the rate of isomerization to the more electrophilic QM , and the chemical reactivity of the quinoids .
	manualset3
180195	7	413921	7	NULL	NULL	0	NULL	 rate of enzymatic formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results substantiate the conclusion that the involvement of the o-quinone / QM pathway in catechol toxicity depends on a combination between the rate of enzymatic formation of the o-quinone , the rate of isomerization to the more electrophilic QM , and the chemical reactivity of the quinoids .
	manualset3
180196	8	413921	7	NULL	NULL	0	NULL	o-quinone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results substantiate the conclusion that the involvement of the o-quinone / QM pathway in catechol toxicity depends on a combination between the rate of enzymatic formation of the o-quinone , the rate of isomerization to the more electrophilic QM , and the chemical reactivity of the quinoids .
	manualset3
180197	9	413921	7	NULL	NULL	0	NULL	 rate of isomerization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results substantiate the conclusion that the involvement of the o-quinone / QM pathway in catechol toxicity depends on a combination between the rate of enzymatic formation of the o-quinone , the rate of isomerization to the more electrophilic QM , and the chemical reactivity of the quinoids .
	manualset3
180198	10	413921	7	NULL	NULL	0	NULL	electrophilic QM	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results substantiate the conclusion that the involvement of the o-quinone / QM pathway in catechol toxicity depends on a combination between the rate of enzymatic formation of the o-quinone , the rate of isomerization to the more electrophilic QM , and the chemical reactivity of the quinoids .
	manualset3
180199	11	413921	7	NULL	NULL	0	NULL	chemical reactivity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results substantiate the conclusion that the involvement of the o-quinone / QM pathway in catechol toxicity depends on a combination between the rate of enzymatic formation of the o-quinone , the rate of isomerization to the more electrophilic QM , and the chemical reactivity of the quinoids .
	manualset3
180200	12	413921	7	NULL	NULL	0	NULL	quinoids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results substantiate the conclusion that the involvement of the o-quinone / QM pathway in catechol toxicity depends on a combination between the rate of enzymatic formation of the o-quinone , the rate of isomerization to the more electrophilic QM , and the chemical reactivity of the quinoids .
	manualset3
180201	1	413922	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest an essential role of the cysteine residue in the export of Pex5p .
	manualset3
180202	2	413922	7	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest an essential role of the cysteine residue in the export of Pex5p .
	manualset3
180203	3	413922	7	NULL	NULL	0	NULL	cysteine residue	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest an essential role of the cysteine residue in the export of Pex5p .
	manualset3
180204	4	413922	7	NULL	NULL	0	NULL	export	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest an essential role of the cysteine residue in the export of Pex5p .
	manualset3
180205	5	413922	7	NULL	NULL	0	NULL	Pex5p	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest an essential role of the cysteine residue in the export of Pex5p .
	manualset3
180206	1	413923	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest no difference in hepatic CYP3A4 activity on menstrual cycle days 2 , 13 , and 21 .
	manualset3
180207	2	413923	7	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest no difference in hepatic CYP3A4 activity on menstrual cycle days 2 , 13 , and 21 .
	manualset3
180208	3	413923	7	NULL	NULL	0	NULL	hepatic CYP3A4 activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest no difference in hepatic CYP3A4 activity on menstrual cycle days 2 , 13 , and 21 .
	manualset3
180209	4	413923	7	NULL	NULL	0	NULL	menstrual cycle days	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest no difference in hepatic CYP3A4 activity on menstrual cycle days 2 , 13 , and 21 .
	manualset3
180210	5	413923	7	NULL	NULL	0	NULL	2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest no difference in hepatic CYP3A4 activity on menstrual cycle days 2 , 13 , and 21 .
	manualset3
180211	6	413923	7	NULL	NULL	0	NULL	13	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest no difference in hepatic CYP3A4 activity on menstrual cycle days 2 , 13 , and 21 .
	manualset3
180212	7	413923	7	NULL	NULL	0	NULL	21	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest no difference in hepatic CYP3A4 activity on menstrual cycle days 2 , 13 , and 21 .
	manualset3
181982	1	413924	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that ( 1 ) PRA is normal in normotensive diabetics , ( 2 ) upright PRA in diabetics with hypertension but no nephropathy is similar to that in essential hypertension , and ( 3 ) patients with diabetes , hypertension , and nephropathy have `` low renin hypertension , '' explaining the virtual absence of malignant hypertension in this group .
	manualset3
181983	2	413924	7	NULL	NULL	0	NULL	PRA	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that ( 1 ) PRA is normal in normotensive diabetics , ( 2 ) upright PRA in diabetics with hypertension but no nephropathy is similar to that in essential hypertension , and ( 3 ) patients with diabetes , hypertension , and nephropathy have `` low renin hypertension , '' explaining the virtual absence of malignant hypertension in this group .
	manualset3
181984	3	413924	7	NULL	NULL	0	NULL	normotensive diabetics	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that ( 1 ) PRA is normal in normotensive diabetics , ( 2 ) upright PRA in diabetics with hypertension but no nephropathy is similar to that in essential hypertension , and ( 3 ) patients with diabetes , hypertension , and nephropathy have `` low renin hypertension , '' explaining the virtual absence of malignant hypertension in this group .
	manualset3
181985	4	413924	7	NULL	NULL	0	NULL	upright PRA	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that ( 1 ) PRA is normal in normotensive diabetics , ( 2 ) upright PRA in diabetics with hypertension but no nephropathy is similar to that in essential hypertension , and ( 3 ) patients with diabetes , hypertension , and nephropathy have `` low renin hypertension , '' explaining the virtual absence of malignant hypertension in this group .
	manualset3
181986	5	413924	7	NULL	NULL	0	NULL	diabetics	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that ( 1 ) PRA is normal in normotensive diabetics , ( 2 ) upright PRA in diabetics with hypertension but no nephropathy is similar to that in essential hypertension , and ( 3 ) patients with diabetes , hypertension , and nephropathy have `` low renin hypertension , '' explaining the virtual absence of malignant hypertension in this group .
	manualset3
181987	6	413924	7	NULL	NULL	0	NULL	hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that ( 1 ) PRA is normal in normotensive diabetics , ( 2 ) upright PRA in diabetics with hypertension but no nephropathy is similar to that in essential hypertension , and ( 3 ) patients with diabetes , hypertension , and nephropathy have `` low renin hypertension , '' explaining the virtual absence of malignant hypertension in this group .
	manualset3
181988	7	413924	7	NULL	NULL	0	NULL	nephropathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that ( 1 ) PRA is normal in normotensive diabetics , ( 2 ) upright PRA in diabetics with hypertension but no nephropathy is similar to that in essential hypertension , and ( 3 ) patients with diabetes , hypertension , and nephropathy have `` low renin hypertension , '' explaining the virtual absence of malignant hypertension in this group .
	manualset3
181989	8	413924	7	NULL	NULL	0	NULL	essential hypertension 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that ( 1 ) PRA is normal in normotensive diabetics , ( 2 ) upright PRA in diabetics with hypertension but no nephropathy is similar to that in essential hypertension , and ( 3 ) patients with diabetes , hypertension , and nephropathy have `` low renin hypertension , '' explaining the virtual absence of malignant hypertension in this group .
	manualset3
181990	9	413924	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that ( 1 ) PRA is normal in normotensive diabetics , ( 2 ) upright PRA in diabetics with hypertension but no nephropathy is similar to that in essential hypertension , and ( 3 ) patients with diabetes , hypertension , and nephropathy have `` low renin hypertension , '' explaining the virtual absence of malignant hypertension in this group .
	manualset3
181991	10	413924	7	NULL	NULL	0	NULL	diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that ( 1 ) PRA is normal in normotensive diabetics , ( 2 ) upright PRA in diabetics with hypertension but no nephropathy is similar to that in essential hypertension , and ( 3 ) patients with diabetes , hypertension , and nephropathy have `` low renin hypertension , '' explaining the virtual absence of malignant hypertension in this group .
	manualset3
181992	11	413924	7	NULL	NULL	0	NULL	hypertension 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that ( 1 ) PRA is normal in normotensive diabetics , ( 2 ) upright PRA in diabetics with hypertension but no nephropathy is similar to that in essential hypertension , and ( 3 ) patients with diabetes , hypertension , and nephropathy have `` low renin hypertension , '' explaining the virtual absence of malignant hypertension in this group .
	manualset3
181993	12	413924	7	NULL	NULL	0	NULL	nephropathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that ( 1 ) PRA is normal in normotensive diabetics , ( 2 ) upright PRA in diabetics with hypertension but no nephropathy is similar to that in essential hypertension , and ( 3 ) patients with diabetes , hypertension , and nephropathy have `` low renin hypertension , '' explaining the virtual absence of malignant hypertension in this group .
	manualset3
181994	13	413924	7	NULL	NULL	0	NULL	low renin hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that ( 1 ) PRA is normal in normotensive diabetics , ( 2 ) upright PRA in diabetics with hypertension but no nephropathy is similar to that in essential hypertension , and ( 3 ) patients with diabetes , hypertension , and nephropathy have `` low renin hypertension , '' explaining the virtual absence of malignant hypertension in this group .
	manualset3
181995	14	413924	7	NULL	NULL	0	NULL	virtual absence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that ( 1 ) PRA is normal in normotensive diabetics , ( 2 ) upright PRA in diabetics with hypertension but no nephropathy is similar to that in essential hypertension , and ( 3 ) patients with diabetes , hypertension , and nephropathy have `` low renin hypertension , '' explaining the virtual absence of malignant hypertension in this group .
	manualset3
181996	15	413924	7	NULL	NULL	0	NULL	malignant hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that ( 1 ) PRA is normal in normotensive diabetics , ( 2 ) upright PRA in diabetics with hypertension but no nephropathy is similar to that in essential hypertension , and ( 3 ) patients with diabetes , hypertension , and nephropathy have `` low renin hypertension , '' explaining the virtual absence of malignant hypertension in this group .
	manualset3
181997	16	413924	7	NULL	NULL	0	NULL	group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that ( 1 ) PRA is normal in normotensive diabetics , ( 2 ) upright PRA in diabetics with hypertension but no nephropathy is similar to that in essential hypertension , and ( 3 ) patients with diabetes , hypertension , and nephropathy have `` low renin hypertension , '' explaining the virtual absence of malignant hypertension in this group .
	manualset3
180213	1	413925	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that , compared to the mouse , spermatogenesis in man is approximately 3.1 times more sensitive to ionizing irradiation .
	manualset3
180214	2	413925	7	NULL	NULL	0	NULL	mouse	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that , compared to the mouse , spermatogenesis in man is approximately 3.1 times more sensitive to ionizing irradiation .
	manualset3
180215	3	413925	7	NULL	NULL	0	NULL	spermatogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that , compared to the mouse , spermatogenesis in man is approximately 3.1 times more sensitive to ionizing irradiation .
	manualset3
180216	4	413925	7	NULL	NULL	0	NULL	 man	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that , compared to the mouse , spermatogenesis in man is approximately 3.1 times more sensitive to ionizing irradiation .
	manualset3
180217	5	413925	7	NULL	NULL	0	NULL	3.1 times	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that , compared to the mouse , spermatogenesis in man is approximately 3.1 times more sensitive to ionizing irradiation .
	manualset3
180218	6	413925	7	NULL	NULL	0	NULL	ionizing irradiation 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that , compared to the mouse , spermatogenesis in man is approximately 3.1 times more sensitive to ionizing irradiation .
	manualset3
180219	1	413926	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that AAs may inhibit platelet aggregation , reduce dispersions of ERP and elevate VFT after coronary occlusion .
	manualset3
180220	2	413926	7	NULL	NULL	0	NULL	 AAs 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that AAs may inhibit platelet aggregation , reduce dispersions of ERP and elevate VFT after coronary occlusion .
	manualset3
180221	3	413926	7	NULL	NULL	0	NULL	platelet aggregation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that AAs may inhibit platelet aggregation , reduce dispersions of ERP and elevate VFT after coronary occlusion .
	manualset3
180222	4	413926	7	NULL	NULL	0	NULL	dispersions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that AAs may inhibit platelet aggregation , reduce dispersions of ERP and elevate VFT after coronary occlusion .
	manualset3
180223	5	413926	7	NULL	NULL	0	NULL	ERP 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that AAs may inhibit platelet aggregation , reduce dispersions of ERP and elevate VFT after coronary occlusion .
	manualset3
180224	6	413926	7	NULL	NULL	0	NULL	VFT	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that AAs may inhibit platelet aggregation , reduce dispersions of ERP and elevate VFT after coronary occlusion .
	manualset3
180225	7	413926	7	NULL	NULL	0	NULL	coronary occlusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that AAs may inhibit platelet aggregation , reduce dispersions of ERP and elevate VFT after coronary occlusion .
	manualset3
180226	1	413927	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that ALA-PDT is a safe and efficient treatment for transplanted patient warts .
	manualset3
180227	2	413927	7	NULL	NULL	0	NULL	ALA-PDT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that ALA-PDT is a safe and efficient treatment for transplanted patient warts .
	manualset3
180228	3	413927	7	NULL	NULL	0	NULL	 treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that ALA-PDT is a safe and efficient treatment for transplanted patient warts .
	manualset3
180229	4	413927	7	NULL	NULL	0	NULL	transplanted patient warts 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that ALA-PDT is a safe and efficient treatment for transplanted patient warts .
	manualset3
180230	1	413928	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that ATA blocks target cell death by inhibition of DNA fragmentation , and further , that chromatin degradation is a cause rather than a result of cell death in CTL-mediated lysis .
	manualset3
180231	2	413928	7	NULL	NULL	0	NULL	ATA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that ATA blocks target cell death by inhibition of DNA fragmentation , and further , that chromatin degradation is a cause rather than a result of cell death in CTL-mediated lysis .
	manualset3
180232	3	413928	7	NULL	NULL	0	NULL	 target cell death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that ATA blocks target cell death by inhibition of DNA fragmentation , and further , that chromatin degradation is a cause rather than a result of cell death in CTL-mediated lysis .
	manualset3
180233	4	413928	7	NULL	NULL	0	NULL	inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that ATA blocks target cell death by inhibition of DNA fragmentation , and further , that chromatin degradation is a cause rather than a result of cell death in CTL-mediated lysis .
	manualset3
180234	5	413928	7	NULL	NULL	0	NULL	DNA fragmentation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that ATA blocks target cell death by inhibition of DNA fragmentation , and further , that chromatin degradation is a cause rather than a result of cell death in CTL-mediated lysis .
	manualset3
180235	6	413928	7	NULL	NULL	0	NULL	chromatin degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that ATA blocks target cell death by inhibition of DNA fragmentation , and further , that chromatin degradation is a cause rather than a result of cell death in CTL-mediated lysis .
	manualset3
180236	7	413928	7	NULL	NULL	0	NULL	result	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that ATA blocks target cell death by inhibition of DNA fragmentation , and further , that chromatin degradation is a cause rather than a result of cell death in CTL-mediated lysis .
	manualset3
180237	8	413928	7	NULL	NULL	0	NULL	cell death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that ATA blocks target cell death by inhibition of DNA fragmentation , and further , that chromatin degradation is a cause rather than a result of cell death in CTL-mediated lysis .
	manualset3
180238	9	413928	7	NULL	NULL	0	NULL	CTL-mediated lysis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that ATA blocks target cell death by inhibition of DNA fragmentation , and further , that chromatin degradation is a cause rather than a result of cell death in CTL-mediated lysis .
	manualset3
180239	1	413929	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that Bulgaria inquinans extract is effective in cutaneous pruritus and erythema , which were probably mediated by inhibiting the release of histamine from mast cells and antagonizing the effect on serotonin .
	manualset3
180240	2	413929	7	NULL	NULL	0	NULL	Bulgaria inquinans extract	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that Bulgaria inquinans extract is effective in cutaneous pruritus and erythema , which were probably mediated by inhibiting the release of histamine from mast cells and antagonizing the effect on serotonin .
	manualset3
180241	3	413929	7	NULL	NULL	0	NULL	cutaneous pruritus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that Bulgaria inquinans extract is effective in cutaneous pruritus and erythema , which were probably mediated by inhibiting the release of histamine from mast cells and antagonizing the effect on serotonin .
	manualset3
180242	4	413929	7	NULL	NULL	0	NULL	erythema	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that Bulgaria inquinans extract is effective in cutaneous pruritus and erythema , which were probably mediated by inhibiting the release of histamine from mast cells and antagonizing the effect on serotonin .
	manualset3
180243	5	413929	7	NULL	NULL	0	NULL	release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that Bulgaria inquinans extract is effective in cutaneous pruritus and erythema , which were probably mediated by inhibiting the release of histamine from mast cells and antagonizing the effect on serotonin .
	manualset3
180244	6	413929	7	NULL	NULL	0	NULL	histamine	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that Bulgaria inquinans extract is effective in cutaneous pruritus and erythema , which were probably mediated by inhibiting the release of histamine from mast cells and antagonizing the effect on serotonin .
	manualset3
180245	7	413929	7	NULL	NULL	0	NULL	mast cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that Bulgaria inquinans extract is effective in cutaneous pruritus and erythema , which were probably mediated by inhibiting the release of histamine from mast cells and antagonizing the effect on serotonin .
	manualset3
180246	8	413929	7	NULL	NULL	0	NULL	effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that Bulgaria inquinans extract is effective in cutaneous pruritus and erythema , which were probably mediated by inhibiting the release of histamine from mast cells and antagonizing the effect on serotonin .
	manualset3
180247	9	413929	7	NULL	NULL	NULL	NULL	serotonin	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results suggest that Bulgaria inquinans extract is effective in cutaneous pruritus and erythema , which were probably mediated by inhibiting the release of histamine from mast cells and antagonizing the effect on serotonin .
	manualset3
180248	1	413930	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that DNA is scavenging free radicals produced within the phospholipid bilayer .
	manualset3
180249	2	413930	7	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that DNA is scavenging free radicals produced within the phospholipid bilayer .
	manualset3
180250	3	413930	7	NULL	NULL	0	NULL	free radicals	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that DNA is scavenging free radicals produced within the phospholipid bilayer .
	manualset3
180251	4	413930	7	NULL	NULL	0	NULL	phospholipid bilayer	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that DNA is scavenging free radicals produced within the phospholipid bilayer .
	manualset3
180524	1	413931	7	NULL	NULL	0	NULL	A23187	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , A23187 led to nucleolus segregation , as revealed by immunocytochemistry using antibodies against DNA and fibrillarin , respectively .
	manualset3
180525	2	413931	7	NULL	NULL	0	NULL	nucleolus segregation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , A23187 led to nucleolus segregation , as revealed by immunocytochemistry using antibodies against DNA and fibrillarin , respectively .
	manualset3
180526	3	413931	7	NULL	NULL	0	NULL	 immunocytochemistry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , A23187 led to nucleolus segregation , as revealed by immunocytochemistry using antibodies against DNA and fibrillarin , respectively .
	manualset3
180527	4	413931	7	NULL	NULL	0	NULL	antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , A23187 led to nucleolus segregation , as revealed by immunocytochemistry using antibodies against DNA and fibrillarin , respectively .
	manualset3
180528	5	413931	7	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , A23187 led to nucleolus segregation , as revealed by immunocytochemistry using antibodies against DNA and fibrillarin , respectively .
	manualset3
180529	6	413931	7	NULL	NULL	0	NULL	fibrillarin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , A23187 led to nucleolus segregation , as revealed by immunocytochemistry using antibodies against DNA and fibrillarin , respectively .
	manualset3
180530	1	413932	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that DNA single-strand breaks were accumulated in freeze-dried spermatozoa preserved under ambient or heat conditions , and then chromatid-type aberrations , especially the chromatid exchanges , were formed via post-replication repair system in zygotes .
	manualset3
180531	2	413932	7	NULL	NULL	0	NULL	DNA single-strand breaks	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that DNA single-strand breaks were accumulated in freeze-dried spermatozoa preserved under ambient or heat conditions , and then chromatid-type aberrations , especially the chromatid exchanges , were formed via post-replication repair system in zygotes .
	manualset3
180532	3	413932	7	NULL	NULL	0	NULL	freeze-dried spermatozoa 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that DNA single-strand breaks were accumulated in freeze-dried spermatozoa preserved under ambient or heat conditions , and then chromatid-type aberrations , especially the chromatid exchanges , were formed via post-replication repair system in zygotes .
	manualset3
180533	4	413932	7	NULL	NULL	0	NULL	 ambient condition	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that DNA single-strand breaks were accumulated in freeze-dried spermatozoa preserved under ambient or heat conditions , and then chromatid-type aberrations , especially the chromatid exchanges , were formed via post-replication repair system in zygotes .
	manualset3
180534	5	413932	7	NULL	NULL	0	NULL	heat conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that DNA single-strand breaks were accumulated in freeze-dried spermatozoa preserved under ambient or heat conditions , and then chromatid-type aberrations , especially the chromatid exchanges , were formed via post-replication repair system in zygotes .
	manualset3
180535	6	413932	7	NULL	NULL	0	NULL	chromatid-type aberrations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that DNA single-strand breaks were accumulated in freeze-dried spermatozoa preserved under ambient or heat conditions , and then chromatid-type aberrations , especially the chromatid exchanges , were formed via post-replication repair system in zygotes .
	manualset3
180536	7	413932	7	NULL	NULL	0	NULL	chromatid exchanges	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that DNA single-strand breaks were accumulated in freeze-dried spermatozoa preserved under ambient or heat conditions , and then chromatid-type aberrations , especially the chromatid exchanges , were formed via post-replication repair system in zygotes .
	manualset3
180537	8	413932	7	NULL	NULL	NULL	NULL	post-replication repair system	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results suggest that DNA single-strand breaks were accumulated in freeze-dried spermatozoa preserved under ambient or heat conditions , and then chromatid-type aberrations , especially the chromatid exchanges , were formed via post-replication repair system in zygotes .
	manualset3
180538	9	413932	7	NULL	NULL	0	NULL	 zygotes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that DNA single-strand breaks were accumulated in freeze-dried spermatozoa preserved under ambient or heat conditions , and then chromatid-type aberrations , especially the chromatid exchanges , were formed via post-replication repair system in zygotes .
	manualset3
180539	1	413933	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that FOP and QM can be used to predict PSE and normal pig meat at different times pm and can replace traditional pH muscle measurements .
	manualset3
180540	2	413933	7	NULL	NULL	0	NULL	FOP	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that FOP and QM can be used to predict PSE and normal pig meat at different times pm and can replace traditional pH muscle measurements .
	manualset3
180541	3	413933	7	NULL	NULL	0	NULL	QM	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that FOP and QM can be used to predict PSE and normal pig meat at different times pm and can replace traditional pH muscle measurements .
	manualset3
180542	4	413933	7	NULL	NULL	0	NULL	PSE pig meat	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that FOP and QM can be used to predict PSE and normal pig meat at different times pm and can replace traditional pH muscle measurements .
	manualset3
180543	5	413933	7	NULL	NULL	0	NULL	normal pig meat	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that FOP and QM can be used to predict PSE and normal pig meat at different times pm and can replace traditional pH muscle measurements .
	manualset3
180544	6	413933	7	NULL	NULL	0	NULL	different times pm	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that FOP and QM can be used to predict PSE and normal pig meat at different times pm and can replace traditional pH muscle measurements .
	manualset3
180545	7	413933	7	NULL	NULL	NULL	NULL	pH muscle measurements	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results suggest that FOP and QM can be used to predict PSE and normal pig meat at different times pm and can replace traditional pH muscle measurements .
	manualset3
180546	1	413934	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that HD-PTP amounts might be regulated both at the transcriptional and post-transcriptional levels .
	manualset3
180547	2	413934	7	NULL	NULL	0	NULL	HD-PTP amounts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that HD-PTP amounts might be regulated both at the transcriptional and post-transcriptional levels .
	manualset3
180548	3	413934	7	NULL	NULL	0	NULL	transcriptional lelvels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that HD-PTP amounts might be regulated both at the transcriptional and post-transcriptional levels .
	manualset3
180549	4	413934	7	NULL	NULL	0	NULL	post-transcriptional levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that HD-PTP amounts might be regulated both at the transcriptional and post-transcriptional levels .
	manualset3
180550	1	413935	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that LYRIC is most likely not a structural component required for TJ formation , but rather is recruited during the maturation of the tight junction complex .
	manualset3
180551	2	413935	7	NULL	NULL	0	NULL	LYRIC	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that LYRIC is most likely not a structural component required for TJ formation , but rather is recruited during the maturation of the tight junction complex .
	manualset3
180552	3	413935	7	NULL	NULL	0	NULL	structural component 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that LYRIC is most likely not a structural component required for TJ formation , but rather is recruited during the maturation of the tight junction complex .
	manualset3
180553	4	413935	7	NULL	NULL	0	NULL	TJ formation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that LYRIC is most likely not a structural component required for TJ formation , but rather is recruited during the maturation of the tight junction complex .
	manualset3
180554	5	413935	7	NULL	NULL	0	NULL	maturation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that LYRIC is most likely not a structural component required for TJ formation , but rather is recruited during the maturation of the tight junction complex .
	manualset3
180555	6	413935	7	NULL	NULL	0	NULL	tight junction complex	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that LYRIC is most likely not a structural component required for TJ formation , but rather is recruited during the maturation of the tight junction complex .
	manualset3
180556	1	413936	7	NULL	NULL	0	NULL	 results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that MRI provides a non-ionising and non-invasive method of demonstrating the early abnormalities of the shoulder associated with obstetrical brachial plexus paralysis , which may prompt orthopaedic correction .
	manualset3
180557	2	413936	7	NULL	NULL	0	NULL	MRI	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that MRI provides a non-ionising and non-invasive method of demonstrating the early abnormalities of the shoulder associated with obstetrical brachial plexus paralysis , which may prompt orthopaedic correction .
	manualset3
180558	3	413936	7	NULL	NULL	0	NULL	non-ionising method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that MRI provides a non-ionising and non-invasive method of demonstrating the early abnormalities of the shoulder associated with obstetrical brachial plexus paralysis , which may prompt orthopaedic correction .
	manualset3
180559	4	413936	7	NULL	NULL	0	NULL	non-invasive method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that MRI provides a non-ionising and non-invasive method of demonstrating the early abnormalities of the shoulder associated with obstetrical brachial plexus paralysis , which may prompt orthopaedic correction .
	manualset3
180560	5	413936	7	NULL	NULL	0	NULL	 early abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that MRI provides a non-ionising and non-invasive method of demonstrating the early abnormalities of the shoulder associated with obstetrical brachial plexus paralysis , which may prompt orthopaedic correction .
	manualset3
180561	6	413936	7	NULL	NULL	0	NULL	shoulder	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that MRI provides a non-ionising and non-invasive method of demonstrating the early abnormalities of the shoulder associated with obstetrical brachial plexus paralysis , which may prompt orthopaedic correction .
	manualset3
180562	7	413936	7	NULL	NULL	0	NULL	obstetrical brachial plexus paralysis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that MRI provides a non-ionising and non-invasive method of demonstrating the early abnormalities of the shoulder associated with obstetrical brachial plexus paralysis , which may prompt orthopaedic correction .
	manualset3
180563	8	413936	7	NULL	NULL	NULL	NULL	orthopaedic correction	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results suggest that MRI provides a non-ionising and non-invasive method of demonstrating the early abnormalities of the shoulder associated with obstetrical brachial plexus paralysis , which may prompt orthopaedic correction .
	manualset3
180564	1	413937	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that MT-PK may have specialized functions in different areas of central nervous system .
	manualset3
180565	2	413937	7	NULL	NULL	0	NULL	MT-PK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that MT-PK may have specialized functions in different areas of central nervous system .
	manualset3
180566	3	413937	7	NULL	NULL	NULL	NULL	specialized functions	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results suggest that MT-PK may have specialized functions in different areas of central nervous system .
	manualset3
180567	4	413937	7	NULL	NULL	0	NULL	different areas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that MT-PK may have specialized functions in different areas of central nervous system .
	manualset3
180568	5	413937	7	NULL	NULL	0	NULL	central nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that MT-PK may have specialized functions in different areas of central nervous system .
	manualset3
180569	1	413938	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that NFLX and CPFX induced DNA single strand breaks ( SSBs ) , and that NFLX-induced SSBs resulted in chromosome aberrations .
	manualset3
180570	2	413938	7	NULL	NULL	0	NULL	NFLX	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that NFLX and CPFX induced DNA single strand breaks ( SSBs ) , and that NFLX-induced SSBs resulted in chromosome aberrations .
	manualset3
180571	3	413938	7	NULL	NULL	0	NULL	CPFX	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that NFLX and CPFX induced DNA single strand breaks ( SSBs ) , and that NFLX-induced SSBs resulted in chromosome aberrations .
	manualset3
180572	4	413938	7	NULL	NULL	0	NULL	DNA single strand breaks ( SSBs )	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that NFLX and CPFX induced DNA single strand breaks ( SSBs ) , and that NFLX-induced SSBs resulted in chromosome aberrations .
	manualset3
180573	5	413938	7	NULL	NULL	NULL	NULL	NFLX-induced SSBs	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results suggest that NFLX and CPFX induced DNA single strand breaks ( SSBs ) , and that NFLX-induced SSBs resulted in chromosome aberrations .
	manualset3
180575	6	413938	7	NULL	NULL	NULL	NULL	chromosome aberrations	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results suggest that NFLX and CPFX induced DNA single strand breaks ( SSBs ) , and that NFLX-induced SSBs resulted in chromosome aberrations .
	manualset3
180576	1	413939	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that Rad54-mediated chromatin remodeling coincides with DNA homology search by the Rad51 presynaptic filament and that this process is facilitated by an interaction of Rad54 with histone H3 .
	manualset3
180577	2	413939	7	NULL	NULL	0	NULL	Rad54-mediated chromatin remodeling 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that Rad54-mediated chromatin remodeling coincides with DNA homology search by the Rad51 presynaptic filament and that this process is facilitated by an interaction of Rad54 with histone H3 .
	manualset3
180578	3	413939	7	NULL	NULL	0	NULL	DNA homology search	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that Rad54-mediated chromatin remodeling coincides with DNA homology search by the Rad51 presynaptic filament and that this process is facilitated by an interaction of Rad54 with histone H3 .
	manualset3
180579	4	413939	7	NULL	NULL	0	NULL	Rad51 presynaptic filament	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that Rad54-mediated chromatin remodeling coincides with DNA homology search by the Rad51 presynaptic filament and that this process is facilitated by an interaction of Rad54 with histone H3 .
	manualset3
180580	5	413939	7	NULL	NULL	0	NULL	process	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that Rad54-mediated chromatin remodeling coincides with DNA homology search by the Rad51 presynaptic filament and that this process is facilitated by an interaction of Rad54 with histone H3 .
	manualset3
180581	6	413939	7	NULL	NULL	0	NULL	interaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that Rad54-mediated chromatin remodeling coincides with DNA homology search by the Rad51 presynaptic filament and that this process is facilitated by an interaction of Rad54 with histone H3 .
	manualset3
180582	7	413939	7	NULL	NULL	0	NULL	Rad54	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that Rad54-mediated chromatin remodeling coincides with DNA homology search by the Rad51 presynaptic filament and that this process is facilitated by an interaction of Rad54 with histone H3 .
	manualset3
180583	8	413939	7	NULL	NULL	0	NULL	histone H3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that Rad54-mediated chromatin remodeling coincides with DNA homology search by the Rad51 presynaptic filament and that this process is facilitated by an interaction of Rad54 with histone H3 .
	manualset3
180584	1	413940	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that Thr192 of Rad9 is the likely phosphorylation site recognized by the FHA1 domain of Rad53 .
	manualset3
180585	2	413940	7	NULL	NULL	0	NULL	Thr192	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that Thr192 of Rad9 is the likely phosphorylation site recognized by the FHA1 domain of Rad53 .
	manualset3
180586	3	413940	7	NULL	NULL	0	NULL	Rad9 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that Thr192 of Rad9 is the likely phosphorylation site recognized by the FHA1 domain of Rad53 .
	manualset3
180587	4	413940	7	NULL	NULL	0	NULL	phosphorylation site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that Thr192 of Rad9 is the likely phosphorylation site recognized by the FHA1 domain of Rad53 .
	manualset3
180588	5	413940	7	NULL	NULL	0	NULL	FHA1 domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that Thr192 of Rad9 is the likely phosphorylation site recognized by the FHA1 domain of Rad53 .
	manualset3
180589	6	413940	7	NULL	NULL	0	NULL	Rad53	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that Thr192 of Rad9 is the likely phosphorylation site recognized by the FHA1 domain of Rad53 .
	manualset3
180590	1	413941	7	NULL	NULL	0	NULL	C-H ... pi interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , C-H ... pi interactions can be found in all the salts analyzed by X-ray diffraction , whereas pi-pi stacking is observed only in the salt containing the phenyltrifluoroborate anion .
	manualset3
180592	2	413941	7	NULL	NULL	0	NULL	salts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , C-H ... pi interactions can be found in all the salts analyzed by X-ray diffraction , whereas pi-pi stacking is observed only in the salt containing the phenyltrifluoroborate anion .
	manualset3
180594	3	413941	7	NULL	NULL	0	NULL	X-ray diffraction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , C-H ... pi interactions can be found in all the salts analyzed by X-ray diffraction , whereas pi-pi stacking is observed only in the salt containing the phenyltrifluoroborate anion .
	manualset3
180595	4	413941	7	NULL	NULL	0	NULL	pi-pi stacking	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , C-H ... pi interactions can be found in all the salts analyzed by X-ray diffraction , whereas pi-pi stacking is observed only in the salt containing the phenyltrifluoroborate anion .
	manualset3
180596	5	413941	7	NULL	NULL	0	NULL	salt	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , C-H ... pi interactions can be found in all the salts analyzed by X-ray diffraction , whereas pi-pi stacking is observed only in the salt containing the phenyltrifluoroborate anion .
	manualset3
180597	6	413941	7	NULL	NULL	0	NULL	phenyltrifluoroborate anion	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , C-H ... pi interactions can be found in all the salts analyzed by X-ray diffraction , whereas pi-pi stacking is observed only in the salt containing the phenyltrifluoroborate anion .
	manualset3
180632	1	413942	7	NULL	NULL	0	NULL	 results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that UK may prevent the mesangial proliferation associated with IgA nephropathy and Henoch-Schnlein purpura nephritis not only by its fibrinolytic action , but also by other mechanisms , such as digestion of the mesangial matrices .
	manualset3
180635	2	413942	7	NULL	NULL	0	NULL	UK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that UK may prevent the mesangial proliferation associated with IgA nephropathy and Henoch-Schnlein purpura nephritis not only by its fibrinolytic action , but also by other mechanisms , such as digestion of the mesangial matrices .
	manualset3
180636	3	413942	7	NULL	NULL	0	NULL	mesangial proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that UK may prevent the mesangial proliferation associated with IgA nephropathy and Henoch-Schnlein purpura nephritis not only by its fibrinolytic action , but also by other mechanisms , such as digestion of the mesangial matrices .
	manualset3
180637	4	413942	7	NULL	NULL	NULL	NULL	IgA nephropathy	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results suggest that UK may prevent the mesangial proliferation associated with IgA nephropathy and Henoch-Schnlein purpura nephritis not only by its fibrinolytic action , but also by other mechanisms , such as digestion of the mesangial matrices .
	manualset3
180638	5	413942	7	NULL	NULL	NULL	NULL	Henoch-Schnlein purpura nephritis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results suggest that UK may prevent the mesangial proliferation associated with IgA nephropathy and Henoch-Schnlein purpura nephritis not only by its fibrinolytic action , but also by other mechanisms , such as digestion of the mesangial matrices .
	manualset3
180639	6	413942	7	NULL	NULL	0	NULL	fibrinolytic action	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that UK may prevent the mesangial proliferation associated with IgA nephropathy and Henoch-Schnlein purpura nephritis not only by its fibrinolytic action , but also by other mechanisms , such as digestion of the mesangial matrices .
	manualset3
180640	7	413942	7	NULL	NULL	0	NULL	mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that UK may prevent the mesangial proliferation associated with IgA nephropathy and Henoch-Schnlein purpura nephritis not only by its fibrinolytic action , but also by other mechanisms , such as digestion of the mesangial matrices .
	manualset3
180641	8	413942	7	NULL	NULL	0	NULL	digestion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that UK may prevent the mesangial proliferation associated with IgA nephropathy and Henoch-Schnlein purpura nephritis not only by its fibrinolytic action , but also by other mechanisms , such as digestion of the mesangial matrices .
	manualset3
180642	9	413942	7	NULL	NULL	0	NULL	mesangial matrices	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that UK may prevent the mesangial proliferation associated with IgA nephropathy and Henoch-Schnlein purpura nephritis not only by its fibrinolytic action , but also by other mechanisms , such as digestion of the mesangial matrices .
	manualset3
180643	1	413943	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that a core mnemonic function of the hippocampus is to bridge representational gaps in our experience .
	manualset3
180644	2	413943	7	NULL	NULL	0	NULL	core mnemonic function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that a core mnemonic function of the hippocampus is to bridge representational gaps in our experience .
	manualset3
180645	3	413943	7	NULL	NULL	0	NULL	hippocampus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that a core mnemonic function of the hippocampus is to bridge representational gaps in our experience .
	manualset3
180646	4	413943	7	NULL	NULL	0	NULL	representational gaps	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that a core mnemonic function of the hippocampus is to bridge representational gaps in our experience .
	manualset3
183555	5	413943	7	NULL	NULL	0	NULL	experience	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that a core mnemonic function of the hippocampus is to bridge representational gaps in our experience .
	manualset3
180647	1	413944	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that a pair of small residues ( presumably flanking the cleavage point ) is required for GPI attachment .
	manualset3
180648	2	413944	7	NULL	NULL	0	NULL	pair of small residues	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that a pair of small residues ( presumably flanking the cleavage point ) is required for GPI attachment .
	manualset3
180649	3	413944	7	NULL	NULL	NULL	NULL	cleavage point	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results suggest that a pair of small residues ( presumably flanking the cleavage point ) is required for GPI attachment .
	manualset3
180650	4	413944	7	NULL	NULL	NULL	NULL	GPI attachment	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results suggest that a pair of small residues ( presumably flanking the cleavage point ) is required for GPI attachment .
	manualset3
180651	1	413945	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that actively growing marine bacteria are physiologically adapted to high internal concentrations of both magnesium and chloride .
	manualset3
180652	2	413945	7	NULL	NULL	0	NULL	actively growing marine bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that actively growing marine bacteria are physiologically adapted to high internal concentrations of both magnesium and chloride .
	manualset3
180653	3	413945	7	NULL	NULL	0	NULL	high internal concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that actively growing marine bacteria are physiologically adapted to high internal concentrations of both magnesium and chloride .
	manualset3
180654	4	413945	7	NULL	NULL	0	NULL	magnesium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that actively growing marine bacteria are physiologically adapted to high internal concentrations of both magnesium and chloride .
	manualset3
180655	5	413945	7	NULL	NULL	0	NULL	chloride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that actively growing marine bacteria are physiologically adapted to high internal concentrations of both magnesium and chloride .
	manualset3
180656	1	413946	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that an enhanced GRK5 expression might play a role in the reduced responsiveness to catecholamines in failing hearts via beta-adrenergic receptor phosphorylation .
	manualset3
180657	2	413946	7	NULL	NULL	0	NULL	enhanced GRK5 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that an enhanced GRK5 expression might play a role in the reduced responsiveness to catecholamines in failing hearts via beta-adrenergic receptor phosphorylation .
	manualset3
180658	3	413946	7	NULL	NULL	0	NULL	reduced responsiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that an enhanced GRK5 expression might play a role in the reduced responsiveness to catecholamines in failing hearts via beta-adrenergic receptor phosphorylation .
	manualset3
180659	4	413946	7	NULL	NULL	0	NULL	catecholamines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that an enhanced GRK5 expression might play a role in the reduced responsiveness to catecholamines in failing hearts via beta-adrenergic receptor phosphorylation .
	manualset3
180660	5	413946	7	NULL	NULL	0	NULL	failing hearts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that an enhanced GRK5 expression might play a role in the reduced responsiveness to catecholamines in failing hearts via beta-adrenergic receptor phosphorylation .
	manualset3
180661	6	413946	7	NULL	NULL	0	NULL	beta-adrenergic receptor phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that an enhanced GRK5 expression might play a role in the reduced responsiveness to catecholamines in failing hearts via beta-adrenergic receptor phosphorylation .
	manualset3
180662	1	413947	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that both HGD and early adenocarcinoma in SSBE and LSBE may occur through similar genetic alterations , whereas there are some clinicopathologic differences between SSBE and LSBE .
	manualset3
180663	2	413947	7	NULL	NULL	0	NULL	HGD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that both HGD and early adenocarcinoma in SSBE and LSBE may occur through similar genetic alterations , whereas there are some clinicopathologic differences between SSBE and LSBE .
	manualset3
180664	3	413947	7	NULL	NULL	0	NULL	early adenocarcinoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that both HGD and early adenocarcinoma in SSBE and LSBE may occur through similar genetic alterations , whereas there are some clinicopathologic differences between SSBE and LSBE .
	manualset3
180665	4	413947	7	NULL	NULL	0	NULL	SSBE	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that both HGD and early adenocarcinoma in SSBE and LSBE may occur through similar genetic alterations , whereas there are some clinicopathologic differences between SSBE and LSBE .
	manualset3
180666	5	413947	7	NULL	NULL	0	NULL	LSBE	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that both HGD and early adenocarcinoma in SSBE and LSBE may occur through similar genetic alterations , whereas there are some clinicopathologic differences between SSBE and LSBE .
	manualset3
180667	6	413947	7	NULL	NULL	0	NULL	genetic alterations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that both HGD and early adenocarcinoma in SSBE and LSBE may occur through similar genetic alterations , whereas there are some clinicopathologic differences between SSBE and LSBE .
	manualset3
180668	7	413947	7	NULL	NULL	0	NULL	clinicopathologic differences 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that both HGD and early adenocarcinoma in SSBE and LSBE may occur through similar genetic alterations , whereas there are some clinicopathologic differences between SSBE and LSBE .
	manualset3
180669	8	413947	7	NULL	NULL	0	NULL	SSBE	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that both HGD and early adenocarcinoma in SSBE and LSBE may occur through similar genetic alterations , whereas there are some clinicopathologic differences between SSBE and LSBE .
	manualset3
180670	9	413947	7	NULL	NULL	0	NULL	LSBE	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that both HGD and early adenocarcinoma in SSBE and LSBE may occur through similar genetic alterations , whereas there are some clinicopathologic differences between SSBE and LSBE .
	manualset3
180671	1	413948	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that bronchodilator reversibility testing should not be used as a rigid basis for treatment decisions with beta2-agonists in COPD patients .
	manualset3
180672	2	413948	7	NULL	NULL	0	NULL	bronchodilator reversibility testing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that bronchodilator reversibility testing should not be used as a rigid basis for treatment decisions with beta2-agonists in COPD patients .
	manualset3
180673	3	413948	7	NULL	NULL	0	NULL	 rigid basis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that bronchodilator reversibility testing should not be used as a rigid basis for treatment decisions with beta2-agonists in COPD patients .
	manualset3
180674	4	413948	7	NULL	NULL	0	NULL	treatment decisions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that bronchodilator reversibility testing should not be used as a rigid basis for treatment decisions with beta2-agonists in COPD patients .
	manualset3
180675	5	413948	7	NULL	NULL	0	NULL	beta2-agonists	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that bronchodilator reversibility testing should not be used as a rigid basis for treatment decisions with beta2-agonists in COPD patients .
	manualset3
180676	6	413948	7	NULL	NULL	0	NULL	COPD patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that bronchodilator reversibility testing should not be used as a rigid basis for treatment decisions with beta2-agonists in COPD patients .
	manualset3
180677	1	413949	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that calcitonin selectively ameliorates enhanced arterial contractility in CCI neuropathic rats , thus leading to its alleviating effect on peripheral circulatory disturbance .
	manualset3
180678	2	413949	7	NULL	NULL	0	NULL	calcitonin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that calcitonin selectively ameliorates enhanced arterial contractility in CCI neuropathic rats , thus leading to its alleviating effect on peripheral circulatory disturbance .
	manualset3
180679	3	413949	7	NULL	NULL	0	NULL	enhanced arterial contractility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that calcitonin selectively ameliorates enhanced arterial contractility in CCI neuropathic rats , thus leading to its alleviating effect on peripheral circulatory disturbance .
	manualset3
180680	4	413949	7	NULL	NULL	0	NULL	CCI neuropathic rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that calcitonin selectively ameliorates enhanced arterial contractility in CCI neuropathic rats , thus leading to its alleviating effect on peripheral circulatory disturbance .
	manualset3
180681	5	413949	7	NULL	NULL	0	NULL	alleviating effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that calcitonin selectively ameliorates enhanced arterial contractility in CCI neuropathic rats , thus leading to its alleviating effect on peripheral circulatory disturbance .
	manualset3
180682	6	413949	7	NULL	NULL	0	NULL	peripheral circulatory disturbance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that calcitonin selectively ameliorates enhanced arterial contractility in CCI neuropathic rats , thus leading to its alleviating effect on peripheral circulatory disturbance .
	manualset3
180683	1	413950	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that citrinin can induce permeability transition by a mechanism that does not involve oxidative damage .
	manualset3
180684	2	413950	7	NULL	NULL	0	NULL	citrinin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that citrinin can induce permeability transition by a mechanism that does not involve oxidative damage .
	manualset3
180685	3	413950	7	NULL	NULL	0	NULL	permeability transition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that citrinin can induce permeability transition by a mechanism that does not involve oxidative damage .
	manualset3
180686	4	413950	7	NULL	NULL	0	NULL	mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that citrinin can induce permeability transition by a mechanism that does not involve oxidative damage .
	manualset3
180687	5	413950	7	NULL	NULL	0	NULL	oxidative damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that citrinin can induce permeability transition by a mechanism that does not involve oxidative damage .
	manualset3
180688	1	413951	7	NULL	NULL	0	NULL	CRI	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , CRI offers advantages of reduced image size and digital storage .
	manualset3
180689	2	413951	7	NULL	NULL	0	NULL	reduced image size	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , CRI offers advantages of reduced image size and digital storage .
	manualset3
180690	3	413951	7	NULL	NULL	NULL	NULL	digital storage	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Additionally , CRI offers advantages of reduced image size and digital storage .
	manualset3
180691	1	413952	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that clinical treatment with 120 mg/day of TOR might be expected to exhibit antiangiogenesis and antimetastasis effects , in addition to inhibition of estrogen-dependent tumor cell growth .
	manualset3
180692	2	413952	7	NULL	NULL	0	NULL	clinical treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that clinical treatment with 120 mg/day of TOR might be expected to exhibit antiangiogenesis and antimetastasis effects , in addition to inhibition of estrogen-dependent tumor cell growth .
	manualset3
180693	3	413952	7	NULL	NULL	0	NULL	120 mg/day	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that clinical treatment with 120 mg/day of TOR might be expected to exhibit antiangiogenesis and antimetastasis effects , in addition to inhibition of estrogen-dependent tumor cell growth .
	manualset3
180694	4	413952	7	NULL	NULL	0	NULL	TOR	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that clinical treatment with 120 mg/day of TOR might be expected to exhibit antiangiogenesis and antimetastasis effects , in addition to inhibition of estrogen-dependent tumor cell growth .
	manualset3
180695	5	413952	7	NULL	NULL	0	NULL	antiangiogenesis effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that clinical treatment with 120 mg/day of TOR might be expected to exhibit antiangiogenesis and antimetastasis effects , in addition to inhibition of estrogen-dependent tumor cell growth .
	manualset3
180696	6	413952	7	NULL	NULL	0	NULL	antimetastasis effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that clinical treatment with 120 mg/day of TOR might be expected to exhibit antiangiogenesis and antimetastasis effects , in addition to inhibition of estrogen-dependent tumor cell growth .
	manualset3
180697	7	413952	7	NULL	NULL	0	NULL	addition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that clinical treatment with 120 mg/day of TOR might be expected to exhibit antiangiogenesis and antimetastasis effects , in addition to inhibition of estrogen-dependent tumor cell growth .
	manualset3
180698	8	413952	7	NULL	NULL	0	NULL	inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that clinical treatment with 120 mg/day of TOR might be expected to exhibit antiangiogenesis and antimetastasis effects , in addition to inhibition of estrogen-dependent tumor cell growth .
	manualset3
180699	9	413952	7	NULL	NULL	0	NULL	estrogen-dependent tumor cell growth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that clinical treatment with 120 mg/day of TOR might be expected to exhibit antiangiogenesis and antimetastasis effects , in addition to inhibition of estrogen-dependent tumor cell growth .
	manualset3
180700	1	413953	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that depression is associated to increase in G protein subunit levels and that the clinical outcome seemed to be the determining factor in further decrease occurring in G protein levels .
	manualset3
180701	2	413953	7	NULL	NULL	0	NULL	depression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that depression is associated to increase in G protein subunit levels and that the clinical outcome seemed to be the determining factor in further decrease occurring in G protein levels .
	manualset3
180702	3	413953	7	NULL	NULL	0	NULL	G protein subunit levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that depression is associated to increase in G protein subunit levels and that the clinical outcome seemed to be the determining factor in further decrease occurring in G protein levels .
	manualset3
180703	4	413953	7	NULL	NULL	0	NULL	clinical outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that depression is associated to increase in G protein subunit levels and that the clinical outcome seemed to be the determining factor in further decrease occurring in G protein levels .
	manualset3
180704	5	413953	7	NULL	NULL	0	NULL	determining factor 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that depression is associated to increase in G protein subunit levels and that the clinical outcome seemed to be the determining factor in further decrease occurring in G protein levels .
	manualset3
180705	6	413953	7	NULL	NULL	0	NULL	G protein levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that depression is associated to increase in G protein subunit levels and that the clinical outcome seemed to be the determining factor in further decrease occurring in G protein levels .
	manualset3
180706	1	413954	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that detection of VanD type resistance is of major importance because it abolishes in vivo glycopeptide activity and allows the emergence of mutants highly resistant to glycopeptides .
	manualset3
180707	2	413954	7	NULL	NULL	0	NULL	detection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that detection of VanD type resistance is of major importance because it abolishes in vivo glycopeptide activity and allows the emergence of mutants highly resistant to glycopeptides .
	manualset3
180708	3	413954	7	NULL	NULL	0	NULL	VanD type resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that detection of VanD type resistance is of major importance because it abolishes in vivo glycopeptide activity and allows the emergence of mutants highly resistant to glycopeptides .
	manualset3
180709	4	413954	7	NULL	NULL	0	NULL	in vivo glycopeptide activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that detection of VanD type resistance is of major importance because it abolishes in vivo glycopeptide activity and allows the emergence of mutants highly resistant to glycopeptides .
	manualset3
180710	5	413954	7	NULL	NULL	0	NULL	emergence of mutants	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that detection of VanD type resistance is of major importance because it abolishes in vivo glycopeptide activity and allows the emergence of mutants highly resistant to glycopeptides .
	manualset3
180711	6	413954	7	NULL	NULL	0	NULL	glycopeptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that detection of VanD type resistance is of major importance because it abolishes in vivo glycopeptide activity and allows the emergence of mutants highly resistant to glycopeptides .
	manualset3
180712	1	413955	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that estrogen status affects tissue distribution of selenium by modulating Sepp1 , as this protein plays a central role in selenium transport .
	manualset3
180713	2	413955	7	NULL	NULL	0	NULL	estrogen status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that estrogen status affects tissue distribution of selenium by modulating Sepp1 , as this protein plays a central role in selenium transport .
	manualset3
180714	3	413955	7	NULL	NULL	0	NULL	tissue distribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that estrogen status affects tissue distribution of selenium by modulating Sepp1 , as this protein plays a central role in selenium transport .
	manualset3
180715	4	413955	7	NULL	NULL	0	NULL	selenium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that estrogen status affects tissue distribution of selenium by modulating Sepp1 , as this protein plays a central role in selenium transport .
	manualset3
180716	5	413955	7	NULL	NULL	NULL	NULL	modulating Sepp1	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results suggest that estrogen status affects tissue distribution of selenium by modulating Sepp1 , as this protein plays a central role in selenium transport .
	manualset3
180717	6	413955	7	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that estrogen status affects tissue distribution of selenium by modulating Sepp1 , as this protein plays a central role in selenium transport .
	manualset3
180718	7	413955	7	NULL	NULL	0	NULL	central role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that estrogen status affects tissue distribution of selenium by modulating Sepp1 , as this protein plays a central role in selenium transport .
	manualset3
180719	8	413955	7	NULL	NULL	0	NULL	selenium transport	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that estrogen status affects tissue distribution of selenium by modulating Sepp1 , as this protein plays a central role in selenium transport .
	manualset3
180720	1	413956	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that exposure to DMN alters bone marrow , particularly the differentiation of effector tumoricidal cells , which renders the host more resistant to metastatic tumor formation .
	manualset3
180721	2	413956	7	NULL	NULL	0	NULL	DMN	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that exposure to DMN alters bone marrow , particularly the differentiation of effector tumoricidal cells , which renders the host more resistant to metastatic tumor formation .
	manualset3
180722	3	413956	7	NULL	NULL	0	NULL	bone marrow	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that exposure to DMN alters bone marrow , particularly the differentiation of effector tumoricidal cells , which renders the host more resistant to metastatic tumor formation .
	manualset3
180723	4	413956	7	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that exposure to DMN alters bone marrow , particularly the differentiation of effector tumoricidal cells , which renders the host more resistant to metastatic tumor formation .
	manualset3
180724	5	413956	7	NULL	NULL	0	NULL	effector tumoricidal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that exposure to DMN alters bone marrow , particularly the differentiation of effector tumoricidal cells , which renders the host more resistant to metastatic tumor formation .
	manualset3
180725	6	413956	7	NULL	NULL	0	NULL	host	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that exposure to DMN alters bone marrow , particularly the differentiation of effector tumoricidal cells , which renders the host more resistant to metastatic tumor formation .
	manualset3
180726	7	413956	7	NULL	NULL	0	NULL	metastatic tumor formation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that exposure to DMN alters bone marrow , particularly the differentiation of effector tumoricidal cells , which renders the host more resistant to metastatic tumor formation .
	manualset3
180727	1	413957	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that feedback inhibition of hepatic lipogenesis in conjunction with post-ER degradation of misfolded apoB proteins can contribute to reduce fat accumulation in the FHBL liver .
	manualset3
180728	2	413957	7	NULL	NULL	NULL	NULL	feedback inhibition	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results suggest that feedback inhibition of hepatic lipogenesis in conjunction with post-ER degradation of misfolded apoB proteins can contribute to reduce fat accumulation in the FHBL liver .
	manualset3
180729	3	413957	7	NULL	NULL	0	NULL	hepatic lipogenesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that feedback inhibition of hepatic lipogenesis in conjunction with post-ER degradation of misfolded apoB proteins can contribute to reduce fat accumulation in the FHBL liver .
	manualset3
180730	4	413957	7	NULL	NULL	0	NULL	conjunction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that feedback inhibition of hepatic lipogenesis in conjunction with post-ER degradation of misfolded apoB proteins can contribute to reduce fat accumulation in the FHBL liver .
	manualset3
180731	5	413957	7	NULL	NULL	0	NULL	post-ER degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that feedback inhibition of hepatic lipogenesis in conjunction with post-ER degradation of misfolded apoB proteins can contribute to reduce fat accumulation in the FHBL liver .
	manualset3
180732	6	413957	7	NULL	NULL	0	NULL	misfolded apoB proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that feedback inhibition of hepatic lipogenesis in conjunction with post-ER degradation of misfolded apoB proteins can contribute to reduce fat accumulation in the FHBL liver .
	manualset3
180733	7	413957	7	NULL	NULL	0	NULL	fat accumulation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that feedback inhibition of hepatic lipogenesis in conjunction with post-ER degradation of misfolded apoB proteins can contribute to reduce fat accumulation in the FHBL liver .
	manualset3
180734	8	413957	7	NULL	NULL	0	NULL	FHBL liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that feedback inhibition of hepatic lipogenesis in conjunction with post-ER degradation of misfolded apoB proteins can contribute to reduce fat accumulation in the FHBL liver .
	manualset3
180735	1	413958	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that first-line fluconazole therapy is effective and well tolerated in patients with AIDS-associated non meningeal cryptococcosis .
	manualset3
180736	2	413958	7	NULL	NULL	0	NULL	first-line fluconazole therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that first-line fluconazole therapy is effective and well tolerated in patients with AIDS-associated non meningeal cryptococcosis .
	manualset3
180737	3	413958	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that first-line fluconazole therapy is effective and well tolerated in patients with AIDS-associated non meningeal cryptococcosis .
	manualset3
180738	4	413958	7	NULL	NULL	0	NULL	AIDS-associated non meningeal cryptococcosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that first-line fluconazole therapy is effective and well tolerated in patients with AIDS-associated non meningeal cryptococcosis .
	manualset3
180739	1	413959	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that gefitinib represses FOXM1 expression via FOXO3a in breast cancer .
	manualset3
180740	2	413959	7	NULL	NULL	0	NULL	gefitinib	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that gefitinib represses FOXM1 expression via FOXO3a in breast cancer .
	manualset3
180741	3	413959	7	NULL	NULL	0	NULL	FOXM1 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that gefitinib represses FOXM1 expression via FOXO3a in breast cancer .
	manualset3
180742	4	413959	7	NULL	NULL	0	NULL	FOXO3a	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that gefitinib represses FOXM1 expression via FOXO3a in breast cancer .
	manualset3
180743	5	413959	7	NULL	NULL	0	NULL	breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that gefitinib represses FOXM1 expression via FOXO3a in breast cancer .
	manualset3
180744	1	413960	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that in MS , OB are monoclonal because they can be stained for gamma heavy chains and for only one light chains .
	manualset3
180745	2	413960	7	NULL	NULL	0	NULL	MS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that in MS , OB are monoclonal because they can be stained for gamma heavy chains and for only one light chains .
	manualset3
180746	3	413960	7	NULL	NULL	0	NULL	OB 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that in MS , OB are monoclonal because they can be stained for gamma heavy chains and for only one light chains .
	manualset3
180747	4	413960	7	NULL	NULL	0	NULL	gamma heavy chains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that in MS , OB are monoclonal because they can be stained for gamma heavy chains and for only one light chains .
	manualset3
180748	5	413960	7	NULL	NULL	0	NULL	one light chains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that in MS , OB are monoclonal because they can be stained for gamma heavy chains and for only one light chains .
	manualset3
180749	1	413961	7	NULL	NULL	0	NULL	 results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that in the presence of heparin , antithrombin III interferes with the catabolism of TFPI mediated via Xa .
	manualset3
180750	2	413961	7	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that in the presence of heparin , antithrombin III interferes with the catabolism of TFPI mediated via Xa .
	manualset3
180751	3	413961	7	NULL	NULL	0	NULL	heparin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that in the presence of heparin , antithrombin III interferes with the catabolism of TFPI mediated via Xa .
	manualset3
180752	4	413961	7	NULL	NULL	0	NULL	antithrombin III	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that in the presence of heparin , antithrombin III interferes with the catabolism of TFPI mediated via Xa .
	manualset3
180753	5	413961	7	NULL	NULL	0	NULL	catabolism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that in the presence of heparin , antithrombin III interferes with the catabolism of TFPI mediated via Xa .
	manualset3
180754	6	413961	7	NULL	NULL	0	NULL	TFPI	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that in the presence of heparin , antithrombin III interferes with the catabolism of TFPI mediated via Xa .
	manualset3
180755	7	413961	7	NULL	NULL	0	NULL	 Xa	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that in the presence of heparin , antithrombin III interferes with the catabolism of TFPI mediated via Xa .
	manualset3
180756	1	413962	7	NULL	NULL	0	NULL	NG-nitro-L : - arginine methyl ester	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , NG-nitro-L : - arginine methyl ester , a nitric oxide synthase inhibitor , failed to regulate COX-2 protein expression but inhibited SP-enhanced COX-2 activity and PGE ( 2 ) production .
	manualset3
180757	2	413962	7	NULL	NULL	0	NULL	nitric oxide synthase inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , NG-nitro-L : - arginine methyl ester , a nitric oxide synthase inhibitor , failed to regulate COX-2 protein expression but inhibited SP-enhanced COX-2 activity and PGE ( 2 ) production .
	manualset3
180758	3	413962	7	NULL	NULL	0	NULL	COX-2 protein expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , NG-nitro-L : - arginine methyl ester , a nitric oxide synthase inhibitor , failed to regulate COX-2 protein expression but inhibited SP-enhanced COX-2 activity and PGE ( 2 ) production .
	manualset3
180759	4	413962	7	NULL	NULL	0	NULL	SP-enhanced COX-2 activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , NG-nitro-L : - arginine methyl ester , a nitric oxide synthase inhibitor , failed to regulate COX-2 protein expression but inhibited SP-enhanced COX-2 activity and PGE ( 2 ) production .
	manualset3
180760	5	413962	7	NULL	NULL	NULL	NULL	PGE ( 2 ) production	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Additionally , NG-nitro-L : - arginine methyl ester , a nitric oxide synthase inhibitor , failed to regulate COX-2 protein expression but inhibited SP-enhanced COX-2 activity and PGE ( 2 ) production .
	manualset3
180761	1	413963	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that iron intake is associated with larger infarct volumes after MCAO in the rat .
	manualset3
180762	2	413963	7	NULL	NULL	0	NULL	 iron intake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that iron intake is associated with larger infarct volumes after MCAO in the rat .
	manualset3
180763	3	413963	7	NULL	NULL	0	NULL	larger infarct volumes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that iron intake is associated with larger infarct volumes after MCAO in the rat .
	manualset3
180764	4	413963	7	NULL	NULL	0	NULL	MCAO	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that iron intake is associated with larger infarct volumes after MCAO in the rat .
	manualset3
180765	5	413963	7	NULL	NULL	0	NULL	 rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that iron intake is associated with larger infarct volumes after MCAO in the rat .
	manualset3
180766	1	413964	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that large-scale genome-wide CNVs and LOH as seen in cancer syndromes are not characteristic findings in PS , although we can not rule out the possibility that newer arrays with a higher number of probes could uncover smaller CNVs not detected in this study .
	manualset3
180767	2	413964	7	NULL	NULL	0	NULL	large-scale genome-wide CNVs	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that large-scale genome-wide CNVs and LOH as seen in cancer syndromes are not characteristic findings in PS , although we can not rule out the possibility that newer arrays with a higher number of probes could uncover smaller CNVs not detected in this study .
	manualset3
180768	3	413964	7	NULL	NULL	0	NULL	LOH	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that large-scale genome-wide CNVs and LOH as seen in cancer syndromes are not characteristic findings in PS , although we can not rule out the possibility that newer arrays with a higher number of probes could uncover smaller CNVs not detected in this study .
	manualset3
180769	4	413964	7	NULL	NULL	0	NULL	cancer syndromes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that large-scale genome-wide CNVs and LOH as seen in cancer syndromes are not characteristic findings in PS , although we can not rule out the possibility that newer arrays with a higher number of probes could uncover smaller CNVs not detected in this study .
	manualset3
180770	5	413964	7	NULL	NULL	0	NULL	 findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that large-scale genome-wide CNVs and LOH as seen in cancer syndromes are not characteristic findings in PS , although we can not rule out the possibility that newer arrays with a higher number of probes could uncover smaller CNVs not detected in this study .
	manualset3
180771	6	413964	7	NULL	NULL	0	NULL	PS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that large-scale genome-wide CNVs and LOH as seen in cancer syndromes are not characteristic findings in PS , although we can not rule out the possibility that newer arrays with a higher number of probes could uncover smaller CNVs not detected in this study .
	manualset3
180772	7	413964	7	NULL	NULL	0	NULL	newer arrays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that large-scale genome-wide CNVs and LOH as seen in cancer syndromes are not characteristic findings in PS , although we can not rule out the possibility that newer arrays with a higher number of probes could uncover smaller CNVs not detected in this study .
	manualset3
180773	8	413964	7	NULL	NULL	0	NULL	higher number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that large-scale genome-wide CNVs and LOH as seen in cancer syndromes are not characteristic findings in PS , although we can not rule out the possibility that newer arrays with a higher number of probes could uncover smaller CNVs not detected in this study .
	manualset3
180774	9	413964	7	NULL	NULL	0	NULL	probes 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that large-scale genome-wide CNVs and LOH as seen in cancer syndromes are not characteristic findings in PS , although we can not rule out the possibility that newer arrays with a higher number of probes could uncover smaller CNVs not detected in this study .
	manualset3
180775	10	413964	7	NULL	NULL	0	NULL	smaller CNVs	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that large-scale genome-wide CNVs and LOH as seen in cancer syndromes are not characteristic findings in PS , although we can not rule out the possibility that newer arrays with a higher number of probes could uncover smaller CNVs not detected in this study .
	manualset3
180776	11	413964	7	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that large-scale genome-wide CNVs and LOH as seen in cancer syndromes are not characteristic findings in PS , although we can not rule out the possibility that newer arrays with a higher number of probes could uncover smaller CNVs not detected in this study .
	manualset3
180777	1	413965	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that low neonatal CORT level serves to protect pups from responding to fear inducing stimuli and attenuate amygdala activation .
	manualset3
180778	2	413965	7	NULL	NULL	0	NULL	low neonatal CORT level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that low neonatal CORT level serves to protect pups from responding to fear inducing stimuli and attenuate amygdala activation .
	manualset3
180779	3	413965	7	NULL	NULL	0	NULL	 pups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that low neonatal CORT level serves to protect pups from responding to fear inducing stimuli and attenuate amygdala activation .
	manualset3
180780	4	413965	7	NULL	NULL	0	NULL	fear inducing stimuli	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that low neonatal CORT level serves to protect pups from responding to fear inducing stimuli and attenuate amygdala activation .
	manualset3
180781	5	413965	7	NULL	NULL	0	NULL	amygdala activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that low neonatal CORT level serves to protect pups from responding to fear inducing stimuli and attenuate amygdala activation .
	manualset3
180782	1	413966	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that low platelet adhesion and spreading are closely related to the low degree of the denaturation of the protein adsorbed onto PMEA .
	manualset3
180783	2	413966	7	NULL	NULL	0	NULL	low platelet adhesion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that low platelet adhesion and spreading are closely related to the low degree of the denaturation of the protein adsorbed onto PMEA .
	manualset3
180784	3	413966	7	NULL	NULL	0	NULL	spreading	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that low platelet adhesion and spreading are closely related to the low degree of the denaturation of the protein adsorbed onto PMEA .
	manualset3
180785	4	413966	7	NULL	NULL	0	NULL	low degree	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that low platelet adhesion and spreading are closely related to the low degree of the denaturation of the protein adsorbed onto PMEA .
	manualset3
180786	5	413966	7	NULL	NULL	0	NULL	denaturation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that low platelet adhesion and spreading are closely related to the low degree of the denaturation of the protein adsorbed onto PMEA .
	manualset3
180787	6	413966	7	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that low platelet adhesion and spreading are closely related to the low degree of the denaturation of the protein adsorbed onto PMEA .
	manualset3
180788	7	413966	7	NULL	NULL	0	NULL	PMEA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that low platelet adhesion and spreading are closely related to the low degree of the denaturation of the protein adsorbed onto PMEA .
	manualset3
180789	1	413967	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that mTOR may play a more important role in the progression of TNBC compared to non-TNBC .
	manualset3
180790	2	413967	7	NULL	NULL	0	NULL	mTOR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that mTOR may play a more important role in the progression of TNBC compared to non-TNBC .
	manualset3
180791	3	413967	7	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that mTOR may play a more important role in the progression of TNBC compared to non-TNBC .
	manualset3
180792	4	413967	7	NULL	NULL	0	NULL	progression 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that mTOR may play a more important role in the progression of TNBC compared to non-TNBC .
	manualset3
180793	5	413967	7	NULL	NULL	0	NULL	TNBC	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that mTOR may play a more important role in the progression of TNBC compared to non-TNBC .
	manualset3
180794	6	413967	7	NULL	NULL	0	NULL	 non-TNBC	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that mTOR may play a more important role in the progression of TNBC compared to non-TNBC .
	manualset3
180795	1	413968	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that mesothelial cells may have a central role not only in pleural fibrosis but also in the onset and progression of IPF .
	manualset3
180796	2	413968	7	NULL	NULL	0	NULL	 mesothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that mesothelial cells may have a central role not only in pleural fibrosis but also in the onset and progression of IPF .
	manualset3
180797	3	413968	7	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that mesothelial cells may have a central role not only in pleural fibrosis but also in the onset and progression of IPF .
	manualset3
180798	4	413968	7	NULL	NULL	0	NULL	pleural fibrosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that mesothelial cells may have a central role not only in pleural fibrosis but also in the onset and progression of IPF .
	manualset3
180799	5	413968	7	NULL	NULL	0	NULL	onset of IPF	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that mesothelial cells may have a central role not only in pleural fibrosis but also in the onset and progression of IPF .
	manualset3
180800	6	413968	7	NULL	NULL	0	NULL	progression of IPF	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that mesothelial cells may have a central role not only in pleural fibrosis but also in the onset and progression of IPF .
	manualset3
180801	1	413969	7	NULL	NULL	0	NULL	 results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that metallic cobalt ( Co ( 0 ) ) is more active than Co ( 2 + ) in the ethanol conversion through dehydrogenation and that Co ( 2 + ) may play a role in the CH ( 4 ) formation .
	manualset3
180802	2	413969	7	NULL	NULL	0	NULL	metallic cobalt ( Co ( 0 ) )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that metallic cobalt ( Co ( 0 ) ) is more active than Co ( 2 + ) in the ethanol conversion through dehydrogenation and that Co ( 2 + ) may play a role in the CH ( 4 ) formation .
	manualset3
180803	3	413969	7	NULL	NULL	NULL	NULL	Co ( 2 + )	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results suggest that metallic cobalt ( Co ( 0 ) ) is more active than Co ( 2 + ) in the ethanol conversion through dehydrogenation and that Co ( 2 + ) may play a role in the CH ( 4 ) formation .
	manualset3
180804	4	413969	7	NULL	NULL	0	NULL	ethanol conversion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that metallic cobalt ( Co ( 0 ) ) is more active than Co ( 2 + ) in the ethanol conversion through dehydrogenation and that Co ( 2 + ) may play a role in the CH ( 4 ) formation .
	manualset3
180805	5	413969	7	NULL	NULL	0	NULL	dehydrogenation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that metallic cobalt ( Co ( 0 ) ) is more active than Co ( 2 + ) in the ethanol conversion through dehydrogenation and that Co ( 2 + ) may play a role in the CH ( 4 ) formation .
	manualset3
180806	6	413969	7	NULL	NULL	0	NULL	Co ( 2 + ) 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that metallic cobalt ( Co ( 0 ) ) is more active than Co ( 2 + ) in the ethanol conversion through dehydrogenation and that Co ( 2 + ) may play a role in the CH ( 4 ) formation .
	manualset3
180807	7	413969	7	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that metallic cobalt ( Co ( 0 ) ) is more active than Co ( 2 + ) in the ethanol conversion through dehydrogenation and that Co ( 2 + ) may play a role in the CH ( 4 ) formation .
	manualset3
180808	8	413969	7	NULL	NULL	0	NULL	CH ( 4 ) formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that metallic cobalt ( Co ( 0 ) ) is more active than Co ( 2 + ) in the ethanol conversion through dehydrogenation and that Co ( 2 + ) may play a role in the CH ( 4 ) formation .
	manualset3
180809	1	413970	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that modern prosociality is not solely the product of an innate psychology , but also reflects norms and institutions that have emerged over the course of human history .
	manualset3
180810	2	413970	7	NULL	NULL	0	NULL	modern prosociality	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that modern prosociality is not solely the product of an innate psychology , but also reflects norms and institutions that have emerged over the course of human history .
	manualset3
180811	3	413970	7	NULL	NULL	0	NULL	product	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that modern prosociality is not solely the product of an innate psychology , but also reflects norms and institutions that have emerged over the course of human history .
	manualset3
180812	4	413970	7	NULL	NULL	0	NULL	innate psychology	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that modern prosociality is not solely the product of an innate psychology , but also reflects norms and institutions that have emerged over the course of human history .
	manualset3
180813	5	413970	7	NULL	NULL	0	NULL	 norms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that modern prosociality is not solely the product of an innate psychology , but also reflects norms and institutions that have emerged over the course of human history .
	manualset3
180814	6	413970	7	NULL	NULL	0	NULL	institutions	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that modern prosociality is not solely the product of an innate psychology , but also reflects norms and institutions that have emerged over the course of human history .
	manualset3
180815	7	413970	7	NULL	NULL	0	NULL	course	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that modern prosociality is not solely the product of an innate psychology , but also reflects norms and institutions that have emerged over the course of human history .
	manualset3
180816	8	413970	7	NULL	NULL	0	NULL	human history	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that modern prosociality is not solely the product of an innate psychology , but also reflects norms and institutions that have emerged over the course of human history .
	manualset3
180817	1	413971	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that normal PrP may be converted to its pathological form at the neuronal plasmalemma or in the extracellular space and , furthermore , that amyloid fibrils are formed following the accumulation and aggregation of subunit proteins at these sites .
	manualset3
180818	2	413971	7	NULL	NULL	0	NULL	normal PrP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that normal PrP may be converted to its pathological form at the neuronal plasmalemma or in the extracellular space and , furthermore , that amyloid fibrils are formed following the accumulation and aggregation of subunit proteins at these sites .
	manualset3
180819	3	413971	7	NULL	NULL	0	NULL	pathological form	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that normal PrP may be converted to its pathological form at the neuronal plasmalemma or in the extracellular space and , furthermore , that amyloid fibrils are formed following the accumulation and aggregation of subunit proteins at these sites .
	manualset3
180820	4	413971	7	NULL	NULL	0	NULL	neuronal plasmalemma	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that normal PrP may be converted to its pathological form at the neuronal plasmalemma or in the extracellular space and , furthermore , that amyloid fibrils are formed following the accumulation and aggregation of subunit proteins at these sites .
	manualset3
180821	5	413971	7	NULL	NULL	0	NULL	extracellular space	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that normal PrP may be converted to its pathological form at the neuronal plasmalemma or in the extracellular space and , furthermore , that amyloid fibrils are formed following the accumulation and aggregation of subunit proteins at these sites .
	manualset3
180822	6	413971	7	NULL	NULL	0	NULL	amyloid fibrils	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that normal PrP may be converted to its pathological form at the neuronal plasmalemma or in the extracellular space and , furthermore , that amyloid fibrils are formed following the accumulation and aggregation of subunit proteins at these sites .
	manualset3
180823	7	413971	7	NULL	NULL	0	NULL	accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that normal PrP may be converted to its pathological form at the neuronal plasmalemma or in the extracellular space and , furthermore , that amyloid fibrils are formed following the accumulation and aggregation of subunit proteins at these sites .
	manualset3
180824	8	413971	7	NULL	NULL	0	NULL	aggregation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that normal PrP may be converted to its pathological form at the neuronal plasmalemma or in the extracellular space and , furthermore , that amyloid fibrils are formed following the accumulation and aggregation of subunit proteins at these sites .
	manualset3
180826	9	413971	7	NULL	NULL	0	NULL	subunit proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that normal PrP may be converted to its pathological form at the neuronal plasmalemma or in the extracellular space and , furthermore , that amyloid fibrils are formed following the accumulation and aggregation of subunit proteins at these sites .
	manualset3
180827	10	413971	7	NULL	NULL	0	NULL	sites	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that normal PrP may be converted to its pathological form at the neuronal plasmalemma or in the extracellular space and , furthermore , that amyloid fibrils are formed following the accumulation and aggregation of subunit proteins at these sites .
	manualset3
180828	1	413972	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that orofacial nociceptive information may be transmitted via P2X ( 3 ) ( + ) afferents to all TBSN and that it may be processed differently in different TBSN .
	manualset3
180829	2	413972	7	NULL	NULL	0	NULL	orofacial nociceptive information	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that orofacial nociceptive information may be transmitted via P2X ( 3 ) ( + ) afferents to all TBSN and that it may be processed differently in different TBSN .
	manualset3
180830	3	413972	7	NULL	NULL	NULL	NULL	P2X ( 3 ) ( + ) afferents	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results suggest that orofacial nociceptive information may be transmitted via P2X ( 3 ) ( + ) afferents to all TBSN and that it may be processed differently in different TBSN .
	manualset3
180831	4	413972	7	NULL	NULL	0	NULL	TBSN	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that orofacial nociceptive information may be transmitted via P2X ( 3 ) ( + ) afferents to all TBSN and that it may be processed differently in different TBSN .
	manualset3
180832	5	413972	7	NULL	NULL	0	NULL	TBSN	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that orofacial nociceptive information may be transmitted via P2X ( 3 ) ( + ) afferents to all TBSN and that it may be processed differently in different TBSN .
	manualset3
180833	1	413973	7	NULL	NULL	0	NULL	forensic sample	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , a forensic sample suspected to contain ricin was analyzed using the presented identification scheme ( data not shown ) .
	manualset3
180834	2	413973	7	NULL	NULL	0	NULL	 ricin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , a forensic sample suspected to contain ricin was analyzed using the presented identification scheme ( data not shown ) .
	manualset3
180835	3	413973	7	NULL	NULL	0	NULL	identification scheme 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , a forensic sample suspected to contain ricin was analyzed using the presented identification scheme ( data not shown ) .
	manualset3
180836	4	413973	7	NULL	NULL	0	NULL	data not shown	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , a forensic sample suspected to contain ricin was analyzed using the presented identification scheme ( data not shown ) .
	manualset3
180837	1	413974	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that oxa-derivatives of vitamin D3 , especially 22-oxa-1 alpha , 25 - ( OH ) 2D3 , should be useful in further studies on the cause and treatment of psoriasis .
	manualset3
180838	2	413974	7	NULL	NULL	0	NULL	oxa-derivatives	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that oxa-derivatives of vitamin D3 , especially 22-oxa-1 alpha , 25 - ( OH ) 2D3 , should be useful in further studies on the cause and treatment of psoriasis .
	manualset3
180839	3	413974	7	NULL	NULL	0	NULL	vitamin D3	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that oxa-derivatives of vitamin D3 , especially 22-oxa-1 alpha , 25 - ( OH ) 2D3 , should be useful in further studies on the cause and treatment of psoriasis .
	manualset3
180840	4	413974	7	NULL	NULL	0	NULL	22-oxa-1 alpha , 25 - ( OH ) 2D3	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that oxa-derivatives of vitamin D3 , especially 22-oxa-1 alpha , 25 - ( OH ) 2D3 , should be useful in further studies on the cause and treatment of psoriasis .
	manualset3
180841	5	413974	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that oxa-derivatives of vitamin D3 , especially 22-oxa-1 alpha , 25 - ( OH ) 2D3 , should be useful in further studies on the cause and treatment of psoriasis .
	manualset3
180842	6	413974	7	NULL	NULL	0	NULL	 treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that oxa-derivatives of vitamin D3 , especially 22-oxa-1 alpha , 25 - ( OH ) 2D3 , should be useful in further studies on the cause and treatment of psoriasis .
	manualset3
180843	7	413974	7	NULL	NULL	0	NULL	psoriasis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that oxa-derivatives of vitamin D3 , especially 22-oxa-1 alpha , 25 - ( OH ) 2D3 , should be useful in further studies on the cause and treatment of psoriasis .
	manualset3
180844	8	413974	7	NULL	NULL	0	NULL	cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that oxa-derivatives of vitamin D3 , especially 22-oxa-1 alpha , 25 - ( OH ) 2D3 , should be useful in further studies on the cause and treatment of psoriasis .
	manualset3
180845	1	413975	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that patients may develop HAMA response after infusion of 111In-Antimyosin Fab , but pathogenic role of HAMA in these patients remains to be studied .
	manualset3
180846	2	413975	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that patients may develop HAMA response after infusion of 111In-Antimyosin Fab , but pathogenic role of HAMA in these patients remains to be studied .
	manualset3
180847	3	413975	7	NULL	NULL	0	NULL	HAMA response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that patients may develop HAMA response after infusion of 111In-Antimyosin Fab , but pathogenic role of HAMA in these patients remains to be studied .
	manualset3
180848	4	413975	7	NULL	NULL	0	NULL	infusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that patients may develop HAMA response after infusion of 111In-Antimyosin Fab , but pathogenic role of HAMA in these patients remains to be studied .
	manualset3
180849	5	413975	7	NULL	NULL	0	NULL	111In-Antimyosin Fab	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that patients may develop HAMA response after infusion of 111In-Antimyosin Fab , but pathogenic role of HAMA in these patients remains to be studied .
	manualset3
180850	6	413975	7	NULL	NULL	0	NULL	pathogenic role	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that patients may develop HAMA response after infusion of 111In-Antimyosin Fab , but pathogenic role of HAMA in these patients remains to be studied .
	manualset3
180851	7	413975	7	NULL	NULL	0	NULL	HAMA	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that patients may develop HAMA response after infusion of 111In-Antimyosin Fab , but pathogenic role of HAMA in these patients remains to be studied .
	manualset3
180852	8	413975	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that patients may develop HAMA response after infusion of 111In-Antimyosin Fab , but pathogenic role of HAMA in these patients remains to be studied .
	manualset3
180853	1	413976	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that postprandial plasma levels of IAPP are not quite sufficient to independently produce satiety .
	manualset3
180854	2	413976	7	NULL	NULL	0	NULL	postprandial plasma levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that postprandial plasma levels of IAPP are not quite sufficient to independently produce satiety .
	manualset3
180855	3	413976	7	NULL	NULL	0	NULL	IAPP	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that postprandial plasma levels of IAPP are not quite sufficient to independently produce satiety .
	manualset3
180856	4	413976	7	NULL	NULL	0	NULL	satiety	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that postprandial plasma levels of IAPP are not quite sufficient to independently produce satiety .
	manualset3
180857	1	413977	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that short life in mice may be caused by n-3 PUFA deficiency and , therefore , the fatty acid may be essential in enjoying a long life .
	manualset3
180858	2	413977	7	NULL	NULL	0	NULL	short life	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that short life in mice may be caused by n-3 PUFA deficiency and , therefore , the fatty acid may be essential in enjoying a long life .
	manualset3
180859	3	413977	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that short life in mice may be caused by n-3 PUFA deficiency and , therefore , the fatty acid may be essential in enjoying a long life .
	manualset3
180860	4	413977	7	NULL	NULL	0	NULL	n-3 PUFA deficiency	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that short life in mice may be caused by n-3 PUFA deficiency and , therefore , the fatty acid may be essential in enjoying a long life .
	manualset3
180861	5	413977	7	NULL	NULL	0	NULL	fatty acid	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that short life in mice may be caused by n-3 PUFA deficiency and , therefore , the fatty acid may be essential in enjoying a long life .
	manualset3
180862	6	413977	7	NULL	NULL	0	NULL	 long life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that short life in mice may be caused by n-3 PUFA deficiency and , therefore , the fatty acid may be essential in enjoying a long life .
	manualset3
180863	1	413978	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that stress levels of cortisol acutely suppress TSH secretion at the pituitary level , with little effect on the TSH pulse generator .
	manualset3
180864	2	413978	7	NULL	NULL	0	NULL	stress levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that stress levels of cortisol acutely suppress TSH secretion at the pituitary level , with little effect on the TSH pulse generator .
	manualset3
180865	3	413978	7	NULL	NULL	0	NULL	cortisol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that stress levels of cortisol acutely suppress TSH secretion at the pituitary level , with little effect on the TSH pulse generator .
	manualset3
180866	4	413978	7	NULL	NULL	0	NULL	TSH secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that stress levels of cortisol acutely suppress TSH secretion at the pituitary level , with little effect on the TSH pulse generator .
	manualset3
180867	5	413978	7	NULL	NULL	0	NULL	pituitary level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that stress levels of cortisol acutely suppress TSH secretion at the pituitary level , with little effect on the TSH pulse generator .
	manualset3
180868	6	413978	7	NULL	NULL	0	NULL	effect 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that stress levels of cortisol acutely suppress TSH secretion at the pituitary level , with little effect on the TSH pulse generator .
	manualset3
180869	7	413978	7	NULL	NULL	0	NULL	TSH pulse generator	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that stress levels of cortisol acutely suppress TSH secretion at the pituitary level , with little effect on the TSH pulse generator .
	manualset3
180870	1	413979	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the ( ( P ) RR ) - dependent activation of prorenin contributes to the pathogenesis of slowly progressive nephropathy in the intact kidney in a rat model of renovascular hypertension .
	manualset3
180871	2	413979	7	NULL	NULL	0	NULL	( ( P ) RR ) - dependent activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the ( ( P ) RR ) - dependent activation of prorenin contributes to the pathogenesis of slowly progressive nephropathy in the intact kidney in a rat model of renovascular hypertension .
	manualset3
180872	3	413979	7	NULL	NULL	0	NULL	prorenin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the ( ( P ) RR ) - dependent activation of prorenin contributes to the pathogenesis of slowly progressive nephropathy in the intact kidney in a rat model of renovascular hypertension .
	manualset3
180873	4	413979	7	NULL	NULL	0	NULL	pathogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the ( ( P ) RR ) - dependent activation of prorenin contributes to the pathogenesis of slowly progressive nephropathy in the intact kidney in a rat model of renovascular hypertension .
	manualset3
180874	5	413979	7	NULL	NULL	0	NULL	slowly progressive nephropathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the ( ( P ) RR ) - dependent activation of prorenin contributes to the pathogenesis of slowly progressive nephropathy in the intact kidney in a rat model of renovascular hypertension .
	manualset3
180875	6	413979	7	NULL	NULL	0	NULL	 intact kidney	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the ( ( P ) RR ) - dependent activation of prorenin contributes to the pathogenesis of slowly progressive nephropathy in the intact kidney in a rat model of renovascular hypertension .
	manualset3
180876	7	413979	7	NULL	NULL	0	NULL	 rat model	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the ( ( P ) RR ) - dependent activation of prorenin contributes to the pathogenesis of slowly progressive nephropathy in the intact kidney in a rat model of renovascular hypertension .
	manualset3
180877	8	413979	7	NULL	NULL	0	NULL	renovascular hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the ( ( P ) RR ) - dependent activation of prorenin contributes to the pathogenesis of slowly progressive nephropathy in the intact kidney in a rat model of renovascular hypertension .
	manualset3
180878	1	413980	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the BMP7-BMPR2-p38-NDRG1 axis plays a critical role in dormancy and recurrence of prostate CSCs in bone and suggest a potential therapeutic utility of BMP7 for recurrent metastatic disease .
	manualset3
180879	2	413980	7	NULL	NULL	0	NULL	BMP7-BMPR2-p38-NDRG1 axis	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the BMP7-BMPR2-p38-NDRG1 axis plays a critical role in dormancy and recurrence of prostate CSCs in bone and suggest a potential therapeutic utility of BMP7 for recurrent metastatic disease .
	manualset3
180880	3	413980	7	NULL	NULL	0	NULL	critical role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the BMP7-BMPR2-p38-NDRG1 axis plays a critical role in dormancy and recurrence of prostate CSCs in bone and suggest a potential therapeutic utility of BMP7 for recurrent metastatic disease .
	manualset3
180881	4	413980	7	NULL	NULL	0	NULL	dormancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the BMP7-BMPR2-p38-NDRG1 axis plays a critical role in dormancy and recurrence of prostate CSCs in bone and suggest a potential therapeutic utility of BMP7 for recurrent metastatic disease .
	manualset3
180882	5	413980	7	NULL	NULL	0	NULL	prostate CSCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the BMP7-BMPR2-p38-NDRG1 axis plays a critical role in dormancy and recurrence of prostate CSCs in bone and suggest a potential therapeutic utility of BMP7 for recurrent metastatic disease .
	manualset3
180883	6	413980	7	NULL	NULL	0	NULL	bone	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the BMP7-BMPR2-p38-NDRG1 axis plays a critical role in dormancy and recurrence of prostate CSCs in bone and suggest a potential therapeutic utility of BMP7 for recurrent metastatic disease .
	manualset3
180884	7	413980	7	NULL	NULL	0	NULL	therapeutic utility	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the BMP7-BMPR2-p38-NDRG1 axis plays a critical role in dormancy and recurrence of prostate CSCs in bone and suggest a potential therapeutic utility of BMP7 for recurrent metastatic disease .
	manualset3
180885	8	413980	7	NULL	NULL	0	NULL	BMP7 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the BMP7-BMPR2-p38-NDRG1 axis plays a critical role in dormancy and recurrence of prostate CSCs in bone and suggest a potential therapeutic utility of BMP7 for recurrent metastatic disease .
	manualset3
180886	9	413980	7	NULL	NULL	0	NULL	metastatic disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the BMP7-BMPR2-p38-NDRG1 axis plays a critical role in dormancy and recurrence of prostate CSCs in bone and suggest a potential therapeutic utility of BMP7 for recurrent metastatic disease .
	manualset3
180887	1	413981	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the CSR-A can be a potential target to prevent lipid accumulation in cells .
	manualset3
180888	2	413981	7	NULL	NULL	0	NULL	CSR-A 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the CSR-A can be a potential target to prevent lipid accumulation in cells .
	manualset3
180889	3	413981	7	NULL	NULL	0	NULL	target	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the CSR-A can be a potential target to prevent lipid accumulation in cells .
	manualset3
180890	4	413981	7	NULL	NULL	NULL	NULL	lipid accumulation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results suggest that the CSR-A can be a potential target to prevent lipid accumulation in cells .
	manualset3
180891	5	413981	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the CSR-A can be a potential target to prevent lipid accumulation in cells .
	manualset3
180892	1	413982	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the LPS-induced NF-kappaB pathways are dependent on both serine and tyrosine phosphorylation of IkappaB-alpha , and that Src TK , such as cSrc and Lck , are key components of the LPS signaling pathway through at least two different mechanisms associated with NF-kappaB activation .
	manualset3
180893	2	413982	7	NULL	NULL	0	NULL	LPS-induced NF-kappaB pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the LPS-induced NF-kappaB pathways are dependent on both serine and tyrosine phosphorylation of IkappaB-alpha , and that Src TK , such as cSrc and Lck , are key components of the LPS signaling pathway through at least two different mechanisms associated with NF-kappaB activation .
	manualset3
180894	3	413982	7	NULL	NULL	0	NULL	serine phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the LPS-induced NF-kappaB pathways are dependent on both serine and tyrosine phosphorylation of IkappaB-alpha , and that Src TK , such as cSrc and Lck , are key components of the LPS signaling pathway through at least two different mechanisms associated with NF-kappaB activation .
	manualset3
180895	4	413982	7	NULL	NULL	0	NULL	tyrosine phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the LPS-induced NF-kappaB pathways are dependent on both serine and tyrosine phosphorylation of IkappaB-alpha , and that Src TK , such as cSrc and Lck , are key components of the LPS signaling pathway through at least two different mechanisms associated with NF-kappaB activation .
	manualset3
180896	5	413982	7	NULL	NULL	0	NULL	IkappaB-alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the LPS-induced NF-kappaB pathways are dependent on both serine and tyrosine phosphorylation of IkappaB-alpha , and that Src TK , such as cSrc and Lck , are key components of the LPS signaling pathway through at least two different mechanisms associated with NF-kappaB activation .
	manualset3
180897	6	413982	7	NULL	NULL	0	NULL	Src TK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the LPS-induced NF-kappaB pathways are dependent on both serine and tyrosine phosphorylation of IkappaB-alpha , and that Src TK , such as cSrc and Lck , are key components of the LPS signaling pathway through at least two different mechanisms associated with NF-kappaB activation .
	manualset3
180898	7	413982	7	NULL	NULL	0	NULL	cSrc	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the LPS-induced NF-kappaB pathways are dependent on both serine and tyrosine phosphorylation of IkappaB-alpha , and that Src TK , such as cSrc and Lck , are key components of the LPS signaling pathway through at least two different mechanisms associated with NF-kappaB activation .
	manualset3
180899	8	413982	7	NULL	NULL	0	NULL	Lck	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the LPS-induced NF-kappaB pathways are dependent on both serine and tyrosine phosphorylation of IkappaB-alpha , and that Src TK , such as cSrc and Lck , are key components of the LPS signaling pathway through at least two different mechanisms associated with NF-kappaB activation .
	manualset3
180900	9	413982	7	NULL	NULL	0	NULL	components	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the LPS-induced NF-kappaB pathways are dependent on both serine and tyrosine phosphorylation of IkappaB-alpha , and that Src TK , such as cSrc and Lck , are key components of the LPS signaling pathway through at least two different mechanisms associated with NF-kappaB activation .
	manualset3
180901	10	413982	7	NULL	NULL	0	NULL	LPS signaling pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the LPS-induced NF-kappaB pathways are dependent on both serine and tyrosine phosphorylation of IkappaB-alpha , and that Src TK , such as cSrc and Lck , are key components of the LPS signaling pathway through at least two different mechanisms associated with NF-kappaB activation .
	manualset3
180902	11	413982	7	NULL	NULL	0	NULL	two different mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the LPS-induced NF-kappaB pathways are dependent on both serine and tyrosine phosphorylation of IkappaB-alpha , and that Src TK , such as cSrc and Lck , are key components of the LPS signaling pathway through at least two different mechanisms associated with NF-kappaB activation .
	manualset3
180903	12	413982	7	NULL	NULL	0	NULL	NF-kappaB activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the LPS-induced NF-kappaB pathways are dependent on both serine and tyrosine phosphorylation of IkappaB-alpha , and that Src TK , such as cSrc and Lck , are key components of the LPS signaling pathway through at least two different mechanisms associated with NF-kappaB activation .
	manualset3
180904	1	413983	7	NULL	NULL	0	NULL	example	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , an example of MO strain and transport study on DyBCO coated conductors is given .
	manualset3
180905	2	413983	7	NULL	NULL	0	NULL	MO strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , an example of MO strain and transport study on DyBCO coated conductors is given .
	manualset3
180906	3	413983	7	NULL	NULL	0	NULL	transport study	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , an example of MO strain and transport study on DyBCO coated conductors is given .
	manualset3
180907	4	413983	7	NULL	NULL	0	NULL	DyBCO coated conductors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , an example of MO strain and transport study on DyBCO coated conductors is given .
	manualset3
180908	1	413984	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the NPs developed in the study can be employed as a potential carrier for oral delivery of heparin .
	manualset3
180909	2	413984	7	NULL	NULL	0	NULL	NPs	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the NPs developed in the study can be employed as a potential carrier for oral delivery of heparin .
	manualset3
180910	3	413984	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the NPs developed in the study can be employed as a potential carrier for oral delivery of heparin .
	manualset3
180911	4	413984	7	NULL	NULL	0	NULL	potential carrier	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the NPs developed in the study can be employed as a potential carrier for oral delivery of heparin .
	manualset3
180912	5	413984	7	NULL	NULL	0	NULL	oral delivery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the NPs developed in the study can be employed as a potential carrier for oral delivery of heparin .
	manualset3
180913	6	413984	7	NULL	NULL	0	NULL	heparin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the NPs developed in the study can be employed as a potential carrier for oral delivery of heparin .
	manualset3
180914	1	413985	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the UT-like immunoreactive substance is produced by neurons in response to brain injury and fear-stress stimuli .
	manualset3
180915	2	413985	7	NULL	NULL	0	NULL	UT-like immunoreactive substance	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the UT-like immunoreactive substance is produced by neurons in response to brain injury and fear-stress stimuli .
	manualset3
180916	3	413985	7	NULL	NULL	0	NULL	neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the UT-like immunoreactive substance is produced by neurons in response to brain injury and fear-stress stimuli .
	manualset3
180917	4	413985	7	NULL	NULL	0	NULL	brain injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the UT-like immunoreactive substance is produced by neurons in response to brain injury and fear-stress stimuli .
	manualset3
180918	5	413985	7	NULL	NULL	0	NULL	fear-stress stimuli	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the UT-like immunoreactive substance is produced by neurons in response to brain injury and fear-stress stimuli .
	manualset3
180919	1	413986	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the antiestrogenic activity of biochanin A and flavone occurs by a mechanism similar to tamoxifen or ICI 182 , 780 .
	manualset3
180920	2	413986	7	NULL	NULL	0	NULL	antiestrogenic activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the antiestrogenic activity of biochanin A and flavone occurs by a mechanism similar to tamoxifen or ICI 182 , 780 .
	manualset3
180921	3	413986	7	NULL	NULL	NULL	NULL	biochanin A	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results suggest that the antiestrogenic activity of biochanin A and flavone occurs by a mechanism similar to tamoxifen or ICI 182 , 780 .
	manualset3
180922	4	413986	7	NULL	NULL	NULL	NULL	flavone	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results suggest that the antiestrogenic activity of biochanin A and flavone occurs by a mechanism similar to tamoxifen or ICI 182 , 780 .
	manualset3
180923	5	413986	7	NULL	NULL	0	NULL	mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the antiestrogenic activity of biochanin A and flavone occurs by a mechanism similar to tamoxifen or ICI 182 , 780 .
	manualset3
180924	6	413986	7	NULL	NULL	0	NULL	 tamoxifen 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the antiestrogenic activity of biochanin A and flavone occurs by a mechanism similar to tamoxifen or ICI 182 , 780 .
	manualset3
180925	7	413986	7	NULL	NULL	0	NULL	ICI 182	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the antiestrogenic activity of biochanin A and flavone occurs by a mechanism similar to tamoxifen or ICI 182 , 780 .
	manualset3
180926	8	413986	7	NULL	NULL	0	NULL	ICI 780	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the antiestrogenic activity of biochanin A and flavone occurs by a mechanism similar to tamoxifen or ICI 182 , 780 .
	manualset3
180927	1	413987	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the co-delivery of CpG ODN adjuvants and antigens in nanospheres is a more efficient approach for immunization than the use of CpG ODN and TT in solution .
	manualset3
180928	2	413987	7	NULL	NULL	0	NULL	co-delivery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the co-delivery of CpG ODN adjuvants and antigens in nanospheres is a more efficient approach for immunization than the use of CpG ODN and TT in solution .
	manualset3
180930	4	413987	7	NULL	NULL	0	NULL	antigens	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the co-delivery of CpG ODN adjuvants and antigens in nanospheres is a more efficient approach for immunization than the use of CpG ODN and TT in solution .
	manualset3
180931	5	413987	7	NULL	NULL	0	NULL	nanospheres	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the co-delivery of CpG ODN adjuvants and antigens in nanospheres is a more efficient approach for immunization than the use of CpG ODN and TT in solution .
	manualset3
180932	6	413987	7	NULL	NULL	0	NULL	approach 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the co-delivery of CpG ODN adjuvants and antigens in nanospheres is a more efficient approach for immunization than the use of CpG ODN and TT in solution .
	manualset3
180933	7	413987	7	NULL	NULL	0	NULL	immunization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the co-delivery of CpG ODN adjuvants and antigens in nanospheres is a more efficient approach for immunization than the use of CpG ODN and TT in solution .
	manualset3
180934	8	413987	7	NULL	NULL	0	NULL	CpG ODN	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the co-delivery of CpG ODN adjuvants and antigens in nanospheres is a more efficient approach for immunization than the use of CpG ODN and TT in solution .
	manualset3
180935	9	413987	7	NULL	NULL	0	NULL	TT	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the co-delivery of CpG ODN adjuvants and antigens in nanospheres is a more efficient approach for immunization than the use of CpG ODN and TT in solution .
	manualset3
180936	10	413987	7	NULL	NULL	0	NULL	solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the co-delivery of CpG ODN adjuvants and antigens in nanospheres is a more efficient approach for immunization than the use of CpG ODN and TT in solution .
	manualset3
180929	3	413988	7	NULL	NULL	NULL	NULL	 CpG ODN adjuvants	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results suggest that the contaminating ALV isolates probably emerged by recombination of ALV-A with endogenous virus sequences before vaccine preparation .
	manualset3
180971	1	413988	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the contaminating ALV isolates probably emerged by recombination of ALV-A with endogenous virus sequences before vaccine preparation .
	manualset3
180972	2	413988	7	NULL	NULL	0	NULL	 contaminating ALV isolates	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the contaminating ALV isolates probably emerged by recombination of ALV-A with endogenous virus sequences before vaccine preparation .
	manualset3
180973	3	413988	7	NULL	NULL	0	NULL	recombination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the contaminating ALV isolates probably emerged by recombination of ALV-A with endogenous virus sequences before vaccine preparation .
	manualset3
180974	4	413988	7	NULL	NULL	0	NULL	ALV-A 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the contaminating ALV isolates probably emerged by recombination of ALV-A with endogenous virus sequences before vaccine preparation .
	manualset3
180976	5	413988	7	NULL	NULL	0	NULL	endogenous virus sequences	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the contaminating ALV isolates probably emerged by recombination of ALV-A with endogenous virus sequences before vaccine preparation .
	manualset3
180979	6	413988	7	NULL	NULL	0	NULL	 vaccine preparation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the contaminating ALV isolates probably emerged by recombination of ALV-A with endogenous virus sequences before vaccine preparation .
	manualset3
180990	1	413989	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the detailed examination of grooming expression and organization is an appropriate tool to measure stress-induced behavioral sensitization and motor functions in animal models of neuropsychiatric disorders such as schizophrenia .
	manualset3
180991	2	413989	7	NULL	NULL	0	NULL	examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the detailed examination of grooming expression and organization is an appropriate tool to measure stress-induced behavioral sensitization and motor functions in animal models of neuropsychiatric disorders such as schizophrenia .
	manualset3
180992	3	413989	7	NULL	NULL	NULL	NULL	grooming expression	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results suggest that the detailed examination of grooming expression and organization is an appropriate tool to measure stress-induced behavioral sensitization and motor functions in animal models of neuropsychiatric disorders such as schizophrenia .
	manualset3
180993	4	413989	7	NULL	NULL	NULL	NULL	organization	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results suggest that the detailed examination of grooming expression and organization is an appropriate tool to measure stress-induced behavioral sensitization and motor functions in animal models of neuropsychiatric disorders such as schizophrenia .
	manualset3
180994	5	413989	7	NULL	NULL	0	NULL	 tool 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the detailed examination of grooming expression and organization is an appropriate tool to measure stress-induced behavioral sensitization and motor functions in animal models of neuropsychiatric disorders such as schizophrenia .
	manualset3
180996	6	413989	7	NULL	NULL	0	NULL	stress-induced behavioral sensitization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the detailed examination of grooming expression and organization is an appropriate tool to measure stress-induced behavioral sensitization and motor functions in animal models of neuropsychiatric disorders such as schizophrenia .
	manualset3
180997	7	413989	7	NULL	NULL	0	NULL	motor functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the detailed examination of grooming expression and organization is an appropriate tool to measure stress-induced behavioral sensitization and motor functions in animal models of neuropsychiatric disorders such as schizophrenia .
	manualset3
180998	8	413989	7	NULL	NULL	0	NULL	animal models	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the detailed examination of grooming expression and organization is an appropriate tool to measure stress-induced behavioral sensitization and motor functions in animal models of neuropsychiatric disorders such as schizophrenia .
	manualset3
180999	9	413989	7	NULL	NULL	0	NULL	neuropsychiatric disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the detailed examination of grooming expression and organization is an appropriate tool to measure stress-induced behavioral sensitization and motor functions in animal models of neuropsychiatric disorders such as schizophrenia .
	manualset3
181000	10	413989	7	NULL	NULL	0	NULL	schizophrenia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the detailed examination of grooming expression and organization is an appropriate tool to measure stress-induced behavioral sensitization and motor functions in animal models of neuropsychiatric disorders such as schizophrenia .
	manualset3
181001	1	413990	7	NULL	NULL	0	NULL	 results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the failure to anchor P1 to the cell wall is due to the lack of cleavage of P1 at the LPXTGX motif .
	manualset3
181002	2	413990	7	NULL	NULL	0	NULL	 failure	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the failure to anchor P1 to the cell wall is due to the lack of cleavage of P1 at the LPXTGX motif .
	manualset3
181003	3	413990	7	NULL	NULL	0	NULL	P1	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the failure to anchor P1 to the cell wall is due to the lack of cleavage of P1 at the LPXTGX motif .
	manualset3
181004	4	413990	7	NULL	NULL	0	NULL	cell wall	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the failure to anchor P1 to the cell wall is due to the lack of cleavage of P1 at the LPXTGX motif .
	manualset3
181005	5	413990	7	NULL	NULL	0	NULL	 lack of cleavage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the failure to anchor P1 to the cell wall is due to the lack of cleavage of P1 at the LPXTGX motif .
	manualset3
181006	6	413990	7	NULL	NULL	0	NULL	P1	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the failure to anchor P1 to the cell wall is due to the lack of cleavage of P1 at the LPXTGX motif .
	manualset3
181007	7	413990	7	NULL	NULL	0	NULL	LPXTGX motif	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the failure to anchor P1 to the cell wall is due to the lack of cleavage of P1 at the LPXTGX motif .
	manualset3
181008	1	413991	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the gap junction protein may have a functional two-domain structure .
	manualset3
181009	2	413991	7	NULL	NULL	0	NULL	gap junction protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the gap junction protein may have a functional two-domain structure .
	manualset3
181010	3	413991	7	NULL	NULL	0	NULL	functional two-domain structure	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the gap junction protein may have a functional two-domain structure .
	manualset3
181011	1	413992	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the inhibitory effect of alpha-tocopherol on lipid peroxidation is due to antioxidant activity rather than the indirect effect of membrane stabilization .
	manualset3
181013	2	413992	7	NULL	NULL	NULL	NULL	inhibitory effect	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results suggest that the inhibitory effect of alpha-tocopherol on lipid peroxidation is due to antioxidant activity rather than the indirect effect of membrane stabilization .
	manualset3
181015	3	413992	7	NULL	NULL	0	NULL	alpha-tocopherol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the inhibitory effect of alpha-tocopherol on lipid peroxidation is due to antioxidant activity rather than the indirect effect of membrane stabilization .
	manualset3
181016	4	413992	7	NULL	NULL	0	NULL	lipid peroxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the inhibitory effect of alpha-tocopherol on lipid peroxidation is due to antioxidant activity rather than the indirect effect of membrane stabilization .
	manualset3
181017	5	413992	7	NULL	NULL	0	NULL	antioxidant activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the inhibitory effect of alpha-tocopherol on lipid peroxidation is due to antioxidant activity rather than the indirect effect of membrane stabilization .
	manualset3
181018	6	413992	7	NULL	NULL	0	NULL	indirect effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the inhibitory effect of alpha-tocopherol on lipid peroxidation is due to antioxidant activity rather than the indirect effect of membrane stabilization .
	manualset3
181019	7	413992	7	NULL	NULL	0	NULL	membrane stabilization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the inhibitory effect of alpha-tocopherol on lipid peroxidation is due to antioxidant activity rather than the indirect effect of membrane stabilization .
	manualset3
181020	1	413993	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the linker has evolved to a length optimal for bringing the two halves of the protein into proper contact with each other , facilitating catalysis .
	manualset3
181021	2	413993	7	NULL	NULL	0	NULL	linker	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the linker has evolved to a length optimal for bringing the two halves of the protein into proper contact with each other , facilitating catalysis .
	manualset3
181022	3	413993	7	NULL	NULL	0	NULL	length	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the linker has evolved to a length optimal for bringing the two halves of the protein into proper contact with each other , facilitating catalysis .
	manualset3
181023	4	413993	7	NULL	NULL	0	NULL	two halves	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the linker has evolved to a length optimal for bringing the two halves of the protein into proper contact with each other , facilitating catalysis .
	manualset3
181024	5	413993	7	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the linker has evolved to a length optimal for bringing the two halves of the protein into proper contact with each other , facilitating catalysis .
	manualset3
181025	6	413993	7	NULL	NULL	0	NULL	contact	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the linker has evolved to a length optimal for bringing the two halves of the protein into proper contact with each other , facilitating catalysis .
	manualset3
181026	7	413993	7	NULL	NULL	0	NULL	 catalysis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the linker has evolved to a length optimal for bringing the two halves of the protein into proper contact with each other , facilitating catalysis .
	manualset3
181027	1	413994	7	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , analysis may suggest that stress resistance is very low in a population or species .
	manualset3
181028	2	413994	7	NULL	NULL	NULL	NULL	stress resistance	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Additionally , analysis may suggest that stress resistance is very low in a population or species .
	manualset3
181029	3	413994	7	NULL	NULL	NULL	NULL	population	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Additionally , analysis may suggest that stress resistance is very low in a population or species .
	manualset3
181030	4	413994	7	NULL	NULL	0	NULL	species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , analysis may suggest that stress resistance is very low in a population or species .
	manualset3
181031	1	413995	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the mucosal adhesive properties of bifidobacteria may be a strain dependent feature , and the mucosal binding of the human bifidobacteria may be more host specific .
	manualset3
181032	2	413995	7	NULL	NULL	0	NULL	mucosal adhesive properties	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the mucosal adhesive properties of bifidobacteria may be a strain dependent feature , and the mucosal binding of the human bifidobacteria may be more host specific .
	manualset3
181033	3	413995	7	NULL	NULL	0	NULL	bifidobacteria 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the mucosal adhesive properties of bifidobacteria may be a strain dependent feature , and the mucosal binding of the human bifidobacteria may be more host specific .
	manualset3
181034	4	413995	7	NULL	NULL	0	NULL	strain dependent feature 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the mucosal adhesive properties of bifidobacteria may be a strain dependent feature , and the mucosal binding of the human bifidobacteria may be more host specific .
	manualset3
181035	5	413995	7	NULL	NULL	0	NULL	mucosal binding 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the mucosal adhesive properties of bifidobacteria may be a strain dependent feature , and the mucosal binding of the human bifidobacteria may be more host specific .
	manualset3
181036	6	413995	7	NULL	NULL	0	NULL	human bifidobacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the mucosal adhesive properties of bifidobacteria may be a strain dependent feature , and the mucosal binding of the human bifidobacteria may be more host specific .
	manualset3
181037	1	413996	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the periodic signal could function as a synchronization signal for the maintenance of reading frame and that codon usage provides a mechanism for manipulation of signal phase .
	manualset3
181038	2	413996	7	NULL	NULL	NULL	NULL	periodic signal	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results suggest that the periodic signal could function as a synchronization signal for the maintenance of reading frame and that codon usage provides a mechanism for manipulation of signal phase .
	manualset3
181039	3	413996	7	NULL	NULL	0	NULL	synchronization signal 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the periodic signal could function as a synchronization signal for the maintenance of reading frame and that codon usage provides a mechanism for manipulation of signal phase .
	manualset3
181040	4	413996	7	NULL	NULL	NULL	NULL	maintenance	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results suggest that the periodic signal could function as a synchronization signal for the maintenance of reading frame and that codon usage provides a mechanism for manipulation of signal phase .
	manualset3
181041	5	413996	7	NULL	NULL	0	NULL	reading frame	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the periodic signal could function as a synchronization signal for the maintenance of reading frame and that codon usage provides a mechanism for manipulation of signal phase .
	manualset3
181042	6	413996	7	NULL	NULL	0	NULL	codon usage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the periodic signal could function as a synchronization signal for the maintenance of reading frame and that codon usage provides a mechanism for manipulation of signal phase .
	manualset3
181043	7	413996	7	NULL	NULL	0	NULL	mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the periodic signal could function as a synchronization signal for the maintenance of reading frame and that codon usage provides a mechanism for manipulation of signal phase .
	manualset3
181044	8	413996	7	NULL	NULL	0	NULL	manipulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the periodic signal could function as a synchronization signal for the maintenance of reading frame and that codon usage provides a mechanism for manipulation of signal phase .
	manualset3
181045	9	413996	7	NULL	NULL	0	NULL	signal phase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the periodic signal could function as a synchronization signal for the maintenance of reading frame and that codon usage provides a mechanism for manipulation of signal phase .
	manualset3
181046	1	413997	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the potent , near-infrared Cy5.5-PSMA inhibitor conjugate may be useful for the detection of prostate tumor cells by optical in vivo imaging .
	manualset3
181047	2	413997	7	NULL	NULL	0	NULL	near-infrared Cy5.5-PSMA inhibitor conjugate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the potent , near-infrared Cy5.5-PSMA inhibitor conjugate may be useful for the detection of prostate tumor cells by optical in vivo imaging .
	manualset3
181048	3	413997	7	NULL	NULL	0	NULL	 detection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the potent , near-infrared Cy5.5-PSMA inhibitor conjugate may be useful for the detection of prostate tumor cells by optical in vivo imaging .
	manualset3
181049	4	413997	7	NULL	NULL	0	NULL	prostate tumor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the potent , near-infrared Cy5.5-PSMA inhibitor conjugate may be useful for the detection of prostate tumor cells by optical in vivo imaging .
	manualset3
181050	5	413997	7	NULL	NULL	0	NULL	optical in vivo imaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the potent , near-infrared Cy5.5-PSMA inhibitor conjugate may be useful for the detection of prostate tumor cells by optical in vivo imaging .
	manualset3
181051	1	413998	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the stimulation of accumulation of small subunit and light-harvesting complex mRNAs by exposure of Pisum seedlings to light is mediated by an increase in transcription rather than by a decrease in RNA degradation .
	manualset3
181052	2	413998	7	NULL	NULL	0	NULL	stimulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the stimulation of accumulation of small subunit and light-harvesting complex mRNAs by exposure of Pisum seedlings to light is mediated by an increase in transcription rather than by a decrease in RNA degradation .
	manualset3
181053	3	413998	7	NULL	NULL	0	NULL	accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the stimulation of accumulation of small subunit and light-harvesting complex mRNAs by exposure of Pisum seedlings to light is mediated by an increase in transcription rather than by a decrease in RNA degradation .
	manualset3
181054	4	413998	7	NULL	NULL	0	NULL	small subunit 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the stimulation of accumulation of small subunit and light-harvesting complex mRNAs by exposure of Pisum seedlings to light is mediated by an increase in transcription rather than by a decrease in RNA degradation .
	manualset3
181055	5	413998	7	NULL	NULL	0	NULL	 light-harvesting complex mRNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the stimulation of accumulation of small subunit and light-harvesting complex mRNAs by exposure of Pisum seedlings to light is mediated by an increase in transcription rather than by a decrease in RNA degradation .
	manualset3
181056	6	413998	7	NULL	NULL	0	NULL	Pisum seedlings	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the stimulation of accumulation of small subunit and light-harvesting complex mRNAs by exposure of Pisum seedlings to light is mediated by an increase in transcription rather than by a decrease in RNA degradation .
	manualset3
181057	7	413998	7	NULL	NULL	0	NULL	 light 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the stimulation of accumulation of small subunit and light-harvesting complex mRNAs by exposure of Pisum seedlings to light is mediated by an increase in transcription rather than by a decrease in RNA degradation .
	manualset3
181058	8	413998	7	NULL	NULL	0	NULL	 increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the stimulation of accumulation of small subunit and light-harvesting complex mRNAs by exposure of Pisum seedlings to light is mediated by an increase in transcription rather than by a decrease in RNA degradation .
	manualset3
181059	9	413998	7	NULL	NULL	0	NULL	transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the stimulation of accumulation of small subunit and light-harvesting complex mRNAs by exposure of Pisum seedlings to light is mediated by an increase in transcription rather than by a decrease in RNA degradation .
	manualset3
181060	10	413998	7	NULL	NULL	0	NULL	decrease	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the stimulation of accumulation of small subunit and light-harvesting complex mRNAs by exposure of Pisum seedlings to light is mediated by an increase in transcription rather than by a decrease in RNA degradation .
	manualset3
181061	11	413998	7	NULL	NULL	0	NULL	RNA degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the stimulation of accumulation of small subunit and light-harvesting complex mRNAs by exposure of Pisum seedlings to light is mediated by an increase in transcription rather than by a decrease in RNA degradation .
	manualset3
181062	1	413999	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the young chimpanzee may be a suitable model for experimental studies of alcoholism .
	manualset3
181063	2	413999	7	NULL	NULL	0	NULL	young chimpanzee	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the young chimpanzee may be a suitable model for experimental studies of alcoholism .
	manualset3
181064	3	413999	7	NULL	NULL	0	NULL	model 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the young chimpanzee may be a suitable model for experimental studies of alcoholism .
	manualset3
181065	4	413999	7	NULL	NULL	0	NULL	experimental studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the young chimpanzee may be a suitable model for experimental studies of alcoholism .
	manualset3
181066	5	413999	7	NULL	NULL	0	NULL	alcoholism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that the young chimpanzee may be a suitable model for experimental studies of alcoholism .
	manualset3
181067	1	414000	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that these ( + ) - benzomorphans may act as agonists at putative sigma heteroreceptors on striatal nerve terminals , or through an indirect mechanism , to modulate dopamine synthesis .
	manualset3
181068	2	414000	7	NULL	NULL	0	NULL	( + ) - benzomorphans	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that these ( + ) - benzomorphans may act as agonists at putative sigma heteroreceptors on striatal nerve terminals , or through an indirect mechanism , to modulate dopamine synthesis .
	manualset3
181069	3	414000	7	NULL	NULL	0	NULL	agonists	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that these ( + ) - benzomorphans may act as agonists at putative sigma heteroreceptors on striatal nerve terminals , or through an indirect mechanism , to modulate dopamine synthesis .
	manualset3
181070	4	414000	7	NULL	NULL	0	NULL	putative sigma heteroreceptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that these ( + ) - benzomorphans may act as agonists at putative sigma heteroreceptors on striatal nerve terminals , or through an indirect mechanism , to modulate dopamine synthesis .
	manualset3
181071	5	414000	7	NULL	NULL	0	NULL	striatal nerve terminals 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that these ( + ) - benzomorphans may act as agonists at putative sigma heteroreceptors on striatal nerve terminals , or through an indirect mechanism , to modulate dopamine synthesis .
	manualset3
181072	6	414000	7	NULL	NULL	0	NULL	indirect mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that these ( + ) - benzomorphans may act as agonists at putative sigma heteroreceptors on striatal nerve terminals , or through an indirect mechanism , to modulate dopamine synthesis .
	manualset3
181073	7	414000	7	NULL	NULL	0	NULL	dopamine synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that these ( + ) - benzomorphans may act as agonists at putative sigma heteroreceptors on striatal nerve terminals , or through an indirect mechanism , to modulate dopamine synthesis .
	manualset3
181074	1	414001	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that this orphan receptor is a member of the opioid receptor family and that dynorphins are endogenous ligands for this receptor .
	manualset3
181075	2	414001	7	NULL	NULL	0	NULL	orphan receptor	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that this orphan receptor is a member of the opioid receptor family and that dynorphins are endogenous ligands for this receptor .
	manualset3
181076	3	414001	7	NULL	NULL	0	NULL	member	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that this orphan receptor is a member of the opioid receptor family and that dynorphins are endogenous ligands for this receptor .
	manualset3
181077	4	414001	7	NULL	NULL	0	NULL	opioid receptor family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that this orphan receptor is a member of the opioid receptor family and that dynorphins are endogenous ligands for this receptor .
	manualset3
181078	5	414001	7	NULL	NULL	0	NULL	dynorphins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that this orphan receptor is a member of the opioid receptor family and that dynorphins are endogenous ligands for this receptor .
	manualset3
181079	6	414001	7	NULL	NULL	0	NULL	endogenous ligands	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that this orphan receptor is a member of the opioid receptor family and that dynorphins are endogenous ligands for this receptor .
	manualset3
181080	7	414001	7	NULL	NULL	0	NULL	receptor	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that this orphan receptor is a member of the opioid receptor family and that dynorphins are endogenous ligands for this receptor .
	manualset3
181081	1	414002	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that unlike many other organ systems in the human body , lung function returns to normal after long term exposure to the removal of gravity .
	manualset3
181082	2	414002	7	NULL	NULL	0	NULL	organ systems	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that unlike many other organ systems in the human body , lung function returns to normal after long term exposure to the removal of gravity .
	manualset3
181083	3	414002	7	NULL	NULL	0	NULL	human body	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that unlike many other organ systems in the human body , lung function returns to normal after long term exposure to the removal of gravity .
	manualset3
181084	4	414002	7	NULL	NULL	0	NULL	 lung function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that unlike many other organ systems in the human body , lung function returns to normal after long term exposure to the removal of gravity .
	manualset3
181085	5	414002	7	NULL	NULL	0	NULL	normal 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that unlike many other organ systems in the human body , lung function returns to normal after long term exposure to the removal of gravity .
	manualset3
181086	6	414002	7	NULL	NULL	0	NULL	long term exposure 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that unlike many other organ systems in the human body , lung function returns to normal after long term exposure to the removal of gravity .
	manualset3
181087	7	414002	7	NULL	NULL	0	NULL	removal of gravity	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that unlike many other organ systems in the human body , lung function returns to normal after long term exposure to the removal of gravity .
	manualset3
181088	1	414003	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that uric acid per se may directly decrease serum 1 , 25 ( OH ) 2-vitamin D3 in patients with gout by inhibiting 1alpha-hydroxylase activity .
	manualset3
181089	2	414003	7	NULL	NULL	0	NULL	 uric acid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that uric acid per se may directly decrease serum 1 , 25 ( OH ) 2-vitamin D3 in patients with gout by inhibiting 1alpha-hydroxylase activity .
	manualset3
181090	3	414003	7	NULL	NULL	0	NULL	serum 1 , 25 ( OH ) 2-vitamin D3	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that uric acid per se may directly decrease serum 1 , 25 ( OH ) 2-vitamin D3 in patients with gout by inhibiting 1alpha-hydroxylase activity .
	manualset3
181091	4	414003	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that uric acid per se may directly decrease serum 1 , 25 ( OH ) 2-vitamin D3 in patients with gout by inhibiting 1alpha-hydroxylase activity .
	manualset3
181092	5	414003	7	NULL	NULL	0	NULL	 gout	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that uric acid per se may directly decrease serum 1 , 25 ( OH ) 2-vitamin D3 in patients with gout by inhibiting 1alpha-hydroxylase activity .
	manualset3
181093	6	414003	7	NULL	NULL	0	NULL	1alpha-hydroxylase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest that uric acid per se may directly decrease serum 1 , 25 ( OH ) 2-vitamin D3 in patients with gout by inhibiting 1alpha-hydroxylase activity .
	manualset3
181094	1	414004	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest theories of partner and parent aggression might gain precision if co-occurrence status were specifically taken into account .
	manualset3
181095	2	414004	7	NULL	NULL	0	NULL	 theories of partner	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest theories of partner and parent aggression might gain precision if co-occurrence status were specifically taken into account .
	manualset3
181096	3	414004	7	NULL	NULL	0	NULL	parent aggression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest theories of partner and parent aggression might gain precision if co-occurrence status were specifically taken into account .
	manualset3
181097	4	414004	7	NULL	NULL	0	NULL	precision	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest theories of partner and parent aggression might gain precision if co-occurrence status were specifically taken into account .
	manualset3
181098	5	414004	7	NULL	NULL	0	NULL	co-occurrence status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest theories of partner and parent aggression might gain precision if co-occurrence status were specifically taken into account .
	manualset3
181099	1	414005	7	NULL	NULL	0	NULL	atrazine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , atrazine adsorbed on sediment ( up to 2.8 ng/g ) and suspended solids was determined ( up to 8 ng/l ) during late spring sampling .
	manualset3
181100	2	414005	7	NULL	NULL	0	NULL	sediment	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , atrazine adsorbed on sediment ( up to 2.8 ng/g ) and suspended solids was determined ( up to 8 ng/l ) during late spring sampling .
	manualset3
181101	3	414005	7	NULL	NULL	0	NULL	2.8 ng/g 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , atrazine adsorbed on sediment ( up to 2.8 ng/g ) and suspended solids was determined ( up to 8 ng/l ) during late spring sampling .
	manualset3
181102	4	414005	7	NULL	NULL	0	NULL	suspended solids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , atrazine adsorbed on sediment ( up to 2.8 ng/g ) and suspended solids was determined ( up to 8 ng/l ) during late spring sampling .
	manualset3
181103	5	414005	7	NULL	NULL	0	NULL	8 ng/l 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , atrazine adsorbed on sediment ( up to 2.8 ng/g ) and suspended solids was determined ( up to 8 ng/l ) during late spring sampling .
	manualset3
181104	6	414005	7	NULL	NULL	0	NULL	late spring sampling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , atrazine adsorbed on sediment ( up to 2.8 ng/g ) and suspended solids was determined ( up to 8 ng/l ) during late spring sampling .
	manualset3
181105	1	414006	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that RSA might act as one of the major scavengers in extracellular fluids under severe oxidative stress .
	manualset3
181106	2	414006	7	NULL	NULL	0	NULL	RSA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that RSA might act as one of the major scavengers in extracellular fluids under severe oxidative stress .
	manualset3
181107	3	414006	7	NULL	NULL	0	NULL	scavengers	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that RSA might act as one of the major scavengers in extracellular fluids under severe oxidative stress .
	manualset3
181108	4	414006	7	NULL	NULL	NULL	NULL	extracellular fluids	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results suggested that RSA might act as one of the major scavengers in extracellular fluids under severe oxidative stress .
	manualset3
181109	5	414006	7	NULL	NULL	0	NULL	severe oxidative stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that RSA might act as one of the major scavengers in extracellular fluids under severe oxidative stress .
	manualset3
181110	1	414007	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that a conformation-dependent epitope play an important role in the development of immunity against blackleg .
	manualset3
181111	2	414007	7	NULL	NULL	0	NULL	conformation-dependent epitope	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that a conformation-dependent epitope play an important role in the development of immunity against blackleg .
	manualset3
181112	3	414007	7	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that a conformation-dependent epitope play an important role in the development of immunity against blackleg .
	manualset3
181113	4	414007	7	NULL	NULL	0	NULL	 development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that a conformation-dependent epitope play an important role in the development of immunity against blackleg .
	manualset3
181114	5	414007	7	NULL	NULL	0	NULL	immunity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that a conformation-dependent epitope play an important role in the development of immunity against blackleg .
	manualset3
181115	6	414007	7	NULL	NULL	0	NULL	blackleg	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that a conformation-dependent epitope play an important role in the development of immunity against blackleg .
	manualset3
181116	1	414008	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that facilitation of the renal kallikrein-kinin system by inhibition of kinin degradation on the luminal side of the renal tubules may effectively prevent hypertension .
	manualset3
181117	2	414008	7	NULL	NULL	0	NULL	 facilitation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that facilitation of the renal kallikrein-kinin system by inhibition of kinin degradation on the luminal side of the renal tubules may effectively prevent hypertension .
	manualset3
181118	3	414008	7	NULL	NULL	0	NULL	renal kallikrein-kinin system	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that facilitation of the renal kallikrein-kinin system by inhibition of kinin degradation on the luminal side of the renal tubules may effectively prevent hypertension .
	manualset3
181119	4	414008	7	NULL	NULL	0	NULL	inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that facilitation of the renal kallikrein-kinin system by inhibition of kinin degradation on the luminal side of the renal tubules may effectively prevent hypertension .
	manualset3
181120	5	414008	7	NULL	NULL	0	NULL	kinin degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that facilitation of the renal kallikrein-kinin system by inhibition of kinin degradation on the luminal side of the renal tubules may effectively prevent hypertension .
	manualset3
181121	6	414008	7	NULL	NULL	0	NULL	luminal side	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that facilitation of the renal kallikrein-kinin system by inhibition of kinin degradation on the luminal side of the renal tubules may effectively prevent hypertension .
	manualset3
181122	7	414008	7	NULL	NULL	0	NULL	renal tubules	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that facilitation of the renal kallikrein-kinin system by inhibition of kinin degradation on the luminal side of the renal tubules may effectively prevent hypertension .
	manualset3
181123	8	414008	7	NULL	NULL	0	NULL	hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that facilitation of the renal kallikrein-kinin system by inhibition of kinin degradation on the luminal side of the renal tubules may effectively prevent hypertension .
	manualset3
181124	1	414009	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that people with low HI titers may become potential carriers of measles and that measurement of pre-exposure HI anti-measles antibody titer is a useful method for selection of candidates to undergo vaccination .
	manualset3
181125	2	414009	7	NULL	NULL	0	NULL	people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that people with low HI titers may become potential carriers of measles and that measurement of pre-exposure HI anti-measles antibody titer is a useful method for selection of candidates to undergo vaccination .
	manualset3
181126	3	414009	7	NULL	NULL	0	NULL	low HI titers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that people with low HI titers may become potential carriers of measles and that measurement of pre-exposure HI anti-measles antibody titer is a useful method for selection of candidates to undergo vaccination .
	manualset3
181127	4	414009	7	NULL	NULL	0	NULL	 potential carriers	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that people with low HI titers may become potential carriers of measles and that measurement of pre-exposure HI anti-measles antibody titer is a useful method for selection of candidates to undergo vaccination .
	manualset3
181128	5	414009	7	NULL	NULL	0	NULL	measles	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that people with low HI titers may become potential carriers of measles and that measurement of pre-exposure HI anti-measles antibody titer is a useful method for selection of candidates to undergo vaccination .
	manualset3
181129	6	414009	7	NULL	NULL	0	NULL	measurement	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that people with low HI titers may become potential carriers of measles and that measurement of pre-exposure HI anti-measles antibody titer is a useful method for selection of candidates to undergo vaccination .
	manualset3
181130	7	414009	7	NULL	NULL	0	NULL	pre-exposure HI anti-measles antibody titer	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that people with low HI titers may become potential carriers of measles and that measurement of pre-exposure HI anti-measles antibody titer is a useful method for selection of candidates to undergo vaccination .
	manualset3
181131	8	414009	7	NULL	NULL	0	NULL	method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that people with low HI titers may become potential carriers of measles and that measurement of pre-exposure HI anti-measles antibody titer is a useful method for selection of candidates to undergo vaccination .
	manualset3
181132	9	414009	7	NULL	NULL	0	NULL	selection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that people with low HI titers may become potential carriers of measles and that measurement of pre-exposure HI anti-measles antibody titer is a useful method for selection of candidates to undergo vaccination .
	manualset3
181133	10	414009	7	NULL	NULL	0	NULL	candidates	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that people with low HI titers may become potential carriers of measles and that measurement of pre-exposure HI anti-measles antibody titer is a useful method for selection of candidates to undergo vaccination .
	manualset3
181134	11	414009	7	NULL	NULL	0	NULL	 vaccination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that people with low HI titers may become potential carriers of measles and that measurement of pre-exposure HI anti-measles antibody titer is a useful method for selection of candidates to undergo vaccination .
	manualset3
181135	1	414010	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that the nonmevalonate pathway and the mevalonate pathway were mainly used for the primary metabolism and the secondary metabolism , respectively , and that both of the two dxs genes were actually transcribed in this strain .
	manualset3
181136	2	414010	7	NULL	NULL	0	NULL	nonmevalonate pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that the nonmevalonate pathway and the mevalonate pathway were mainly used for the primary metabolism and the secondary metabolism , respectively , and that both of the two dxs genes were actually transcribed in this strain .
	manualset3
181137	3	414010	7	NULL	NULL	0	NULL	mevalonate pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that the nonmevalonate pathway and the mevalonate pathway were mainly used for the primary metabolism and the secondary metabolism , respectively , and that both of the two dxs genes were actually transcribed in this strain .
	manualset3
181138	4	414010	7	NULL	NULL	0	NULL	primary metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that the nonmevalonate pathway and the mevalonate pathway were mainly used for the primary metabolism and the secondary metabolism , respectively , and that both of the two dxs genes were actually transcribed in this strain .
	manualset3
181139	5	414010	7	NULL	NULL	0	NULL	secondary metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that the nonmevalonate pathway and the mevalonate pathway were mainly used for the primary metabolism and the secondary metabolism , respectively , and that both of the two dxs genes were actually transcribed in this strain .
	manualset3
181140	6	414010	7	NULL	NULL	0	NULL	two dxs genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that the nonmevalonate pathway and the mevalonate pathway were mainly used for the primary metabolism and the secondary metabolism , respectively , and that both of the two dxs genes were actually transcribed in this strain .
	manualset3
181141	7	414010	7	NULL	NULL	0	NULL	strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that the nonmevalonate pathway and the mevalonate pathway were mainly used for the primary metabolism and the secondary metabolism , respectively , and that both of the two dxs genes were actually transcribed in this strain .
	manualset3
181142	1	414011	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support a model for IDDM in which Thl-cell-mediated tissue damage is initially regulated by Valpha24JalphaQ + T cells producing both cytokines ; the loss of their capacity to secrete IL-4 is correlated with IDDM .
	manualset3
181143	2	414011	7	NULL	NULL	0	NULL	model	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support a model for IDDM in which Thl-cell-mediated tissue damage is initially regulated by Valpha24JalphaQ + T cells producing both cytokines ; the loss of their capacity to secrete IL-4 is correlated with IDDM .
	manualset3
181144	3	414011	7	NULL	NULL	0	NULL	IDDM	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support a model for IDDM in which Thl-cell-mediated tissue damage is initially regulated by Valpha24JalphaQ + T cells producing both cytokines ; the loss of their capacity to secrete IL-4 is correlated with IDDM .
	manualset3
181145	4	414011	7	NULL	NULL	0	NULL	Thl-cell-mediated tissue damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support a model for IDDM in which Thl-cell-mediated tissue damage is initially regulated by Valpha24JalphaQ + T cells producing both cytokines ; the loss of their capacity to secrete IL-4 is correlated with IDDM .
	manualset3
181146	5	414011	7	NULL	NULL	0	NULL	Valpha24JalphaQ + T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support a model for IDDM in which Thl-cell-mediated tissue damage is initially regulated by Valpha24JalphaQ + T cells producing both cytokines ; the loss of their capacity to secrete IL-4 is correlated with IDDM .
	manualset3
181147	6	414011	7	NULL	NULL	0	NULL	cytokines	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support a model for IDDM in which Thl-cell-mediated tissue damage is initially regulated by Valpha24JalphaQ + T cells producing both cytokines ; the loss of their capacity to secrete IL-4 is correlated with IDDM .
	manualset3
181148	7	414011	7	NULL	NULL	0	NULL	loss 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support a model for IDDM in which Thl-cell-mediated tissue damage is initially regulated by Valpha24JalphaQ + T cells producing both cytokines ; the loss of their capacity to secrete IL-4 is correlated with IDDM .
	manualset3
181149	8	414011	7	NULL	NULL	0	NULL	IL-4 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support a model for IDDM in which Thl-cell-mediated tissue damage is initially regulated by Valpha24JalphaQ + T cells producing both cytokines ; the loss of their capacity to secrete IL-4 is correlated with IDDM .
	manualset3
181150	9	414011	7	NULL	NULL	0	NULL	IDDM	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support a model for IDDM in which Thl-cell-mediated tissue damage is initially regulated by Valpha24JalphaQ + T cells producing both cytokines ; the loss of their capacity to secrete IL-4 is correlated with IDDM .
	manualset3
181151	10	414011	7	NULL	NULL	0	NULL	capacity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support a model for IDDM in which Thl-cell-mediated tissue damage is initially regulated by Valpha24JalphaQ + T cells producing both cytokines ; the loss of their capacity to secrete IL-4 is correlated with IDDM .
	manualset3
181152	1	414012	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support efforts to treat human colorectal cancer by pharmacological inhibition of the Wnt / - catenin pathway .
	manualset3
181153	2	414012	7	NULL	NULL	0	NULL	human colorectal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support efforts to treat human colorectal cancer by pharmacological inhibition of the Wnt / - catenin pathway .
	manualset3
181154	3	414012	7	NULL	NULL	0	NULL	 pharmacological inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support efforts to treat human colorectal cancer by pharmacological inhibition of the Wnt / - catenin pathway .
	manualset3
181155	4	414012	7	NULL	NULL	0	NULL	Wnt / - catenin pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support efforts to treat human colorectal cancer by pharmacological inhibition of the Wnt / - catenin pathway .
	manualset3
181156	1	414013	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support previous findings indicating that during word recognition , the RH activates a broader range of related meanings than the LH , including alternate meanings of ambiguous words .
	manualset3
181157	2	414013	7	NULL	NULL	0	NULL	previous findings	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support previous findings indicating that during word recognition , the RH activates a broader range of related meanings than the LH , including alternate meanings of ambiguous words .
	manualset3
181158	3	414013	7	NULL	NULL	0	NULL	word recognition	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support previous findings indicating that during word recognition , the RH activates a broader range of related meanings than the LH , including alternate meanings of ambiguous words .
	manualset3
181159	4	414013	7	NULL	NULL	0	NULL	RH 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support previous findings indicating that during word recognition , the RH activates a broader range of related meanings than the LH , including alternate meanings of ambiguous words .
	manualset3
181160	5	414013	7	NULL	NULL	0	NULL	broader range	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support previous findings indicating that during word recognition , the RH activates a broader range of related meanings than the LH , including alternate meanings of ambiguous words .
	manualset3
181161	7	414013	7	NULL	NULL	NULL	NULL	LH	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results support previous findings indicating that during word recognition , the RH activates a broader range of related meanings than the LH , including alternate meanings of ambiguous words .
	manualset3
181162	6	414013	7	NULL	NULL	0	NULL	 related meanings	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support previous findings indicating that during word recognition , the RH activates a broader range of related meanings than the LH , including alternate meanings of ambiguous words .
	manualset3
181163	8	414013	7	NULL	NULL	0	NULL	alternate meanings	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support previous findings indicating that during word recognition , the RH activates a broader range of related meanings than the LH , including alternate meanings of ambiguous words .
	manualset3
181164	9	414013	7	NULL	NULL	0	NULL	ambiguous words	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support previous findings indicating that during word recognition , the RH activates a broader range of related meanings than the LH , including alternate meanings of ambiguous words .
	manualset3
181165	1	414014	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support the association of rs30250202 and rs3025039 , and specific VEGF haplotypes , with altered VEGF serum levels , although the exact functional mechanisms remain to be elucidated .
	manualset3
181166	2	414014	7	NULL	NULL	0	NULL	association	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support the association of rs30250202 and rs3025039 , and specific VEGF haplotypes , with altered VEGF serum levels , although the exact functional mechanisms remain to be elucidated .
	manualset3
181167	3	414014	7	NULL	NULL	0	NULL	rs30250202	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support the association of rs30250202 and rs3025039 , and specific VEGF haplotypes , with altered VEGF serum levels , although the exact functional mechanisms remain to be elucidated .
	manualset3
181168	4	414014	7	NULL	NULL	0	NULL	rs3025039	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support the association of rs30250202 and rs3025039 , and specific VEGF haplotypes , with altered VEGF serum levels , although the exact functional mechanisms remain to be elucidated .
	manualset3
181169	5	414014	7	NULL	NULL	0	NULL	 specific VEGF haplotypes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support the association of rs30250202 and rs3025039 , and specific VEGF haplotypes , with altered VEGF serum levels , although the exact functional mechanisms remain to be elucidated .
	manualset3
181170	6	414014	7	NULL	NULL	0	NULL	altered VEGF serum levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support the association of rs30250202 and rs3025039 , and specific VEGF haplotypes , with altered VEGF serum levels , although the exact functional mechanisms remain to be elucidated .
	manualset3
181171	7	414014	7	NULL	NULL	0	NULL	functional mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support the association of rs30250202 and rs3025039 , and specific VEGF haplotypes , with altered VEGF serum levels , although the exact functional mechanisms remain to be elucidated .
	manualset3
181172	1	414015	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support the hypothesis that brain glycogen could decrease with prolonged exhaustive exercise .
	manualset3
181173	2	414015	7	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support the hypothesis that brain glycogen could decrease with prolonged exhaustive exercise .
	manualset3
181174	3	414015	7	NULL	NULL	0	NULL	brain glycogen	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support the hypothesis that brain glycogen could decrease with prolonged exhaustive exercise .
	manualset3
181175	4	414015	7	NULL	NULL	0	NULL	prolonged exhaustive exercise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support the hypothesis that brain glycogen could decrease with prolonged exhaustive exercise .
	manualset3
181176	1	414016	7	NULL	NULL	0	NULL	Comparative study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative study of ribonucleic acid of the bacillus Proteus & of the fixed L-forms derived from it ) .
	manualset3
181177	2	414016	7	NULL	NULL	0	NULL	ribonucleic acid	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative study of ribonucleic acid of the bacillus Proteus & of the fixed L-forms derived from it ) .
	manualset3
181178	3	414016	7	NULL	NULL	0	NULL	bacillus Proteus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative study of ribonucleic acid of the bacillus Proteus & of the fixed L-forms derived from it ) .
	manualset3
181179	4	414016	7	NULL	NULL	0	NULL	fixed L-forms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative study of ribonucleic acid of the bacillus Proteus & of the fixed L-forms derived from it ) .
	manualset3
181180	1	414017	7	NULL	NULL	0	NULL	c-Mpl ligands	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , c-Mpl ligands may have a role in improving apheresis yields when administered to normal platelet donors .
	manualset3
181181	2	414017	7	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , c-Mpl ligands may have a role in improving apheresis yields when administered to normal platelet donors .
	manualset3
181182	3	414017	7	NULL	NULL	0	NULL	apheresis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , c-Mpl ligands may have a role in improving apheresis yields when administered to normal platelet donors .
	manualset3
181183	4	414017	7	NULL	NULL	0	NULL	normal platelet donors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , c-Mpl ligands may have a role in improving apheresis yields when administered to normal platelet donors .
	manualset3
181184	1	414018	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support the notion that perforated synapses involving double-headed dendritic spines represent a structural modification related to enhanced synaptic efficacy .
	manualset3
181185	2	414018	7	NULL	NULL	0	NULL	notion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support the notion that perforated synapses involving double-headed dendritic spines represent a structural modification related to enhanced synaptic efficacy .
	manualset3
181186	3	414018	7	NULL	NULL	0	NULL	synapses	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support the notion that perforated synapses involving double-headed dendritic spines represent a structural modification related to enhanced synaptic efficacy .
	manualset3
181187	4	414018	7	NULL	NULL	0	NULL	double-headed dendritic spines	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support the notion that perforated synapses involving double-headed dendritic spines represent a structural modification related to enhanced synaptic efficacy .
	manualset3
181188	5	414018	7	NULL	NULL	0	NULL	structural modification	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support the notion that perforated synapses involving double-headed dendritic spines represent a structural modification related to enhanced synaptic efficacy .
	manualset3
181189	6	414018	7	NULL	NULL	0	NULL	synaptic efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support the notion that perforated synapses involving double-headed dendritic spines represent a structural modification related to enhanced synaptic efficacy .
	manualset3
181190	1	414019	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support the possibility that induction of lysosomal protease synthesis may underlie burn-induced increases in muscle proteolysis .
	manualset3
181191	2	414019	7	NULL	NULL	0	NULL	possibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support the possibility that induction of lysosomal protease synthesis may underlie burn-induced increases in muscle proteolysis .
	manualset3
181192	3	414019	7	NULL	NULL	0	NULL	induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support the possibility that induction of lysosomal protease synthesis may underlie burn-induced increases in muscle proteolysis .
	manualset3
181193	4	414019	7	NULL	NULL	0	NULL	lysosomal protease synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support the possibility that induction of lysosomal protease synthesis may underlie burn-induced increases in muscle proteolysis .
	manualset3
181194	5	414019	7	NULL	NULL	0	NULL	 burn-induced increases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support the possibility that induction of lysosomal protease synthesis may underlie burn-induced increases in muscle proteolysis .
	manualset3
181195	6	414019	7	NULL	NULL	0	NULL	muscle proteolysis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support the possibility that induction of lysosomal protease synthesis may underlie burn-induced increases in muscle proteolysis .
	manualset3
181196	1	414020	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results underscore the value of CR2-TAg mice for characterizing normal NE cell biology and tumorigenesis .
	manualset3
181197	2	414020	7	NULL	NULL	0	NULL	value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results underscore the value of CR2-TAg mice for characterizing normal NE cell biology and tumorigenesis .
	manualset3
181198	3	414020	7	NULL	NULL	0	NULL	CR2-TAg mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results underscore the value of CR2-TAg mice for characterizing normal NE cell biology and tumorigenesis .
	manualset3
181199	4	414020	7	NULL	NULL	0	NULL	normal NE cell biology 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These results underscore the value of CR2-TAg mice for characterizing normal NE cell biology and tumorigenesis .
	manualset3
181200	5	414020	7	NULL	NULL	0	NULL	tumorigenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results underscore the value of CR2-TAg mice for characterizing normal NE cell biology and tumorigenesis .
	manualset3
181201	1	414021	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results validate D-PCa-2 as a transcript with high tissue specificity and with a potential application in the diagnosis of PCa .
	manualset3
181202	2	414021	7	NULL	NULL	0	NULL	D-PCa-2 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These results validate D-PCa-2 as a transcript with high tissue specificity and with a potential application in the diagnosis of PCa .
	manualset3
181203	3	414021	7	NULL	NULL	0	NULL	 transcript	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These results validate D-PCa-2 as a transcript with high tissue specificity and with a potential application in the diagnosis of PCa .
	manualset3
181204	4	414021	7	NULL	NULL	0	NULL	high tissue specificity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results validate D-PCa-2 as a transcript with high tissue specificity and with a potential application in the diagnosis of PCa .
	manualset3
181205	5	414021	7	NULL	NULL	0	NULL	potential application	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results validate D-PCa-2 as a transcript with high tissue specificity and with a potential application in the diagnosis of PCa .
	manualset3
181206	6	414021	7	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results validate D-PCa-2 as a transcript with high tissue specificity and with a potential application in the diagnosis of PCa .
	manualset3
181207	7	414021	7	NULL	NULL	0	NULL	PCa	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results validate D-PCa-2 as a transcript with high tissue specificity and with a potential application in the diagnosis of PCa .
	manualset3
181208	1	414022	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results validate the use of cryopreservation in preserving the viability and functionality of PEG-encapsulated BMP2-transduced MSCs .
	manualset3
181209	2	414022	7	NULL	NULL	0	NULL	cryopreservation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results validate the use of cryopreservation in preserving the viability and functionality of PEG-encapsulated BMP2-transduced MSCs .
	manualset3
181210	3	414022	7	NULL	NULL	0	NULL	viability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results validate the use of cryopreservation in preserving the viability and functionality of PEG-encapsulated BMP2-transduced MSCs .
	manualset3
181211	4	414022	7	NULL	NULL	0	NULL	functionality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results validate the use of cryopreservation in preserving the viability and functionality of PEG-encapsulated BMP2-transduced MSCs .
	manualset3
181212	5	414022	7	NULL	NULL	0	NULL	PEG-encapsulated BMP2-transduced MSCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results validate the use of cryopreservation in preserving the viability and functionality of PEG-encapsulated BMP2-transduced MSCs .
	manualset3
181213	1	414023	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results were compared to 11 patients who received steroid therapy for ACR .
	manualset3
181214	2	414023	7	NULL	NULL	0	NULL	11 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These results were compared to 11 patients who received steroid therapy for ACR .
	manualset3
181215	3	414023	7	NULL	NULL	0	NULL	steroid therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These results were compared to 11 patients who received steroid therapy for ACR .
	manualset3
181216	4	414023	7	NULL	NULL	0	NULL	ACR	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results were compared to 11 patients who received steroid therapy for ACR .
	manualset3
181217	1	414024	7	NULL	NULL	0	NULL	gaps	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , gaps in the literature are identified and recommendations are made for clinical research that could be done to provide more definitive evidence for the use of C2 or other LSSs in monitoring liver transplant patients .
	manualset3
181218	2	414024	7	NULL	NULL	0	NULL	literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , gaps in the literature are identified and recommendations are made for clinical research that could be done to provide more definitive evidence for the use of C2 or other LSSs in monitoring liver transplant patients .
	manualset3
181219	3	414024	7	NULL	NULL	0	NULL	recommendations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , gaps in the literature are identified and recommendations are made for clinical research that could be done to provide more definitive evidence for the use of C2 or other LSSs in monitoring liver transplant patients .
	manualset3
181220	4	414024	7	NULL	NULL	0	NULL	clinical research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , gaps in the literature are identified and recommendations are made for clinical research that could be done to provide more definitive evidence for the use of C2 or other LSSs in monitoring liver transplant patients .
	manualset3
181221	5	414024	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , gaps in the literature are identified and recommendations are made for clinical research that could be done to provide more definitive evidence for the use of C2 or other LSSs in monitoring liver transplant patients .
	manualset3
181222	6	414024	7	NULL	NULL	0	NULL	use of C2	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , gaps in the literature are identified and recommendations are made for clinical research that could be done to provide more definitive evidence for the use of C2 or other LSSs in monitoring liver transplant patients .
	manualset3
181223	7	414024	7	NULL	NULL	0	NULL	LSSs	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , gaps in the literature are identified and recommendations are made for clinical research that could be done to provide more definitive evidence for the use of C2 or other LSSs in monitoring liver transplant patients .
	manualset3
181224	8	414024	7	NULL	NULL	0	NULL	liver transplant patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , gaps in the literature are identified and recommendations are made for clinical research that could be done to provide more definitive evidence for the use of C2 or other LSSs in monitoring liver transplant patients .
	manualset3
181225	1	414025	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results were verified in three independently isolated clones of Rat 1 fibroblasts transfected with the HIR delta CT cDNA .
	manualset3
181226	2	414025	7	NULL	NULL	0	NULL	three independently isolated clones	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results were verified in three independently isolated clones of Rat 1 fibroblasts transfected with the HIR delta CT cDNA .
	manualset3
181227	3	414025	7	NULL	NULL	0	NULL	Rat 1 fibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results were verified in three independently isolated clones of Rat 1 fibroblasts transfected with the HIR delta CT cDNA .
	manualset3
181228	4	414025	7	NULL	NULL	0	NULL	HIR delta CT cDNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These results were verified in three independently isolated clones of Rat 1 fibroblasts transfected with the HIR delta CT cDNA .
	manualset3
181229	1	414026	7	NULL	NULL	0	NULL	ribozymes	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These ribozymes have cleaved the target RNAs in culture system ( in vitro ) and developed in vivo system .
	manualset3
181230	2	414026	7	NULL	NULL	0	NULL	target RNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These ribozymes have cleaved the target RNAs in culture system ( in vitro ) and developed in vivo system .
	manualset3
181231	3	414026	7	NULL	NULL	0	NULL	culture system ( in vitro )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These ribozymes have cleaved the target RNAs in culture system ( in vitro ) and developed in vivo system .
	manualset3
181232	4	414026	7	NULL	NULL	0	NULL	in vivo system	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These ribozymes have cleaved the target RNAs in culture system ( in vitro ) and developed in vivo system .
	manualset3
181233	1	414027	7	NULL	NULL	0	NULL	risk calculations	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These risk calculations indicate that the Chernobyl fallout can not explain the entire increase in thyroid cancers in France , and that it is improbable that an epidemiological study could demonstrate such an excess .
	manualset3
181234	2	414027	7	NULL	NULL	0	NULL	Chernobyl fallout	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These risk calculations indicate that the Chernobyl fallout can not explain the entire increase in thyroid cancers in France , and that it is improbable that an epidemiological study could demonstrate such an excess .
	manualset3
181235	3	414027	7	NULL	NULL	0	NULL	increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These risk calculations indicate that the Chernobyl fallout can not explain the entire increase in thyroid cancers in France , and that it is improbable that an epidemiological study could demonstrate such an excess .
	manualset3
181236	4	414027	7	NULL	NULL	0	NULL	thyroid cancers 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These risk calculations indicate that the Chernobyl fallout can not explain the entire increase in thyroid cancers in France , and that it is improbable that an epidemiological study could demonstrate such an excess .
	manualset3
181237	5	414027	7	NULL	NULL	0	NULL	France	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	These risk calculations indicate that the Chernobyl fallout can not explain the entire increase in thyroid cancers in France , and that it is improbable that an epidemiological study could demonstrate such an excess .
	manualset3
181238	6	414027	7	NULL	NULL	0	NULL	epidemiological study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These risk calculations indicate that the Chernobyl fallout can not explain the entire increase in thyroid cancers in France , and that it is improbable that an epidemiological study could demonstrate such an excess .
	manualset3
181239	1	414028	7	NULL	NULL	0	NULL	 rne mutants	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These rne mutants grew nearly normally in the mukB + genetic background .
	manualset3
181240	2	414028	7	NULL	NULL	0	NULL	mukB + genetic background	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These rne mutants grew nearly normally in the mukB + genetic background .
	manualset3
181241	1	414029	7	NULL	NULL	0	NULL	similarities	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These similarities-and the conditions ' differences-provide a context for reviewing the articles in this issue about clinical approaches to children with gender dysphoria , in relation to assessment , intervention , and ethics .
	manualset3
181242	2	414029	7	NULL	NULL	0	NULL	conditions 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These similarities-and the conditions ' differences-provide a context for reviewing the articles in this issue about clinical approaches to children with gender dysphoria , in relation to assessment , intervention , and ethics .
	manualset3
181243	3	414029	7	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These similarities-and the conditions ' differences-provide a context for reviewing the articles in this issue about clinical approaches to children with gender dysphoria , in relation to assessment , intervention , and ethics .
	manualset3
181244	4	414029	7	NULL	NULL	0	NULL	context	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These similarities-and the conditions ' differences-provide a context for reviewing the articles in this issue about clinical approaches to children with gender dysphoria , in relation to assessment , intervention , and ethics .
	manualset3
181245	5	414029	7	NULL	NULL	0	NULL	articles	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These similarities-and the conditions ' differences-provide a context for reviewing the articles in this issue about clinical approaches to children with gender dysphoria , in relation to assessment , intervention , and ethics .
	manualset3
181246	6	414029	7	NULL	NULL	0	NULL	 issue	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These similarities-and the conditions ' differences-provide a context for reviewing the articles in this issue about clinical approaches to children with gender dysphoria , in relation to assessment , intervention , and ethics .
	manualset3
181247	7	414029	7	NULL	NULL	NULL	NULL	clinical approaches	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These similarities-and the conditions ' differences-provide a context for reviewing the articles in this issue about clinical approaches to children with gender dysphoria , in relation to assessment , intervention , and ethics .
	manualset3
181248	8	414029	7	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These similarities-and the conditions ' differences-provide a context for reviewing the articles in this issue about clinical approaches to children with gender dysphoria , in relation to assessment , intervention , and ethics .
	manualset3
181249	9	414029	7	NULL	NULL	0	NULL	gender dysphoria	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These similarities-and the conditions ' differences-provide a context for reviewing the articles in this issue about clinical approaches to children with gender dysphoria , in relation to assessment , intervention , and ethics .
	manualset3
181250	10	414029	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These similarities-and the conditions ' differences-provide a context for reviewing the articles in this issue about clinical approaches to children with gender dysphoria , in relation to assessment , intervention , and ethics .
	manualset3
181251	11	414029	7	NULL	NULL	0	NULL	assessment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These similarities-and the conditions ' differences-provide a context for reviewing the articles in this issue about clinical approaches to children with gender dysphoria , in relation to assessment , intervention , and ethics .
	manualset3
181252	12	414029	7	NULL	NULL	0	NULL	intervention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These similarities-and the conditions ' differences-provide a context for reviewing the articles in this issue about clinical approaches to children with gender dysphoria , in relation to assessment , intervention , and ethics .
	manualset3
181253	13	414029	7	NULL	NULL	0	NULL	ethics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These similarities-and the conditions ' differences-provide a context for reviewing the articles in this issue about clinical approaches to children with gender dysphoria , in relation to assessment , intervention , and ethics .
	manualset3
183837	14	414029	7	NULL	NULL	0	NULL	reviewing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These similarities-and the conditions ' differences-provide a context for reviewing the articles in this issue about clinical approaches to children with gender dysphoria , in relation to assessment , intervention , and ethics .
	manualset3
181254	1	414030	7	NULL	NULL	0	NULL	species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These species may be found in water , food and in the intestinal tract of chickens .
	manualset3
181255	2	414030	7	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These species may be found in water , food and in the intestinal tract of chickens .
	manualset3
181256	3	414030	7	NULL	NULL	0	NULL	food 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	These species may be found in water , food and in the intestinal tract of chickens .
	manualset3
181257	4	414030	7	NULL	NULL	0	NULL	 intestinal tract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These species may be found in water , food and in the intestinal tract of chickens .
	manualset3
181258	5	414030	7	NULL	NULL	0	NULL	chickens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These species may be found in water , food and in the intestinal tract of chickens .
	manualset3
181998	1	414031	7	NULL	NULL	0	NULL	hormonal homeostasis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , hormonal homeostasis seemed to be affected in nrt2 , which displays priming of salicylic acid signaling and concomitant irregular functioning of the jasmonic acid and abscisic acid pathways upon infection .
	manualset3
181999	2	414031	7	NULL	NULL	0	NULL	nrt2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , hormonal homeostasis seemed to be affected in nrt2 , which displays priming of salicylic acid signaling and concomitant irregular functioning of the jasmonic acid and abscisic acid pathways upon infection .
	manualset3
182000	3	414031	7	NULL	NULL	0	NULL	priming 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , hormonal homeostasis seemed to be affected in nrt2 , which displays priming of salicylic acid signaling and concomitant irregular functioning of the jasmonic acid and abscisic acid pathways upon infection .
	manualset3
182001	4	414031	7	NULL	NULL	0	NULL	salicylic acid signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , hormonal homeostasis seemed to be affected in nrt2 , which displays priming of salicylic acid signaling and concomitant irregular functioning of the jasmonic acid and abscisic acid pathways upon infection .
	manualset3
182002	5	414031	7	NULL	NULL	0	NULL	irregular functioning	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , hormonal homeostasis seemed to be affected in nrt2 , which displays priming of salicylic acid signaling and concomitant irregular functioning of the jasmonic acid and abscisic acid pathways upon infection .
	manualset3
182003	6	414031	7	NULL	NULL	0	NULL	jasmonic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , hormonal homeostasis seemed to be affected in nrt2 , which displays priming of salicylic acid signaling and concomitant irregular functioning of the jasmonic acid and abscisic acid pathways upon infection .
	manualset3
182004	7	414031	7	NULL	NULL	0	NULL	abscisic acid pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , hormonal homeostasis seemed to be affected in nrt2 , which displays priming of salicylic acid signaling and concomitant irregular functioning of the jasmonic acid and abscisic acid pathways upon infection .
	manualset3
182005	8	414031	7	NULL	NULL	0	NULL	 infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , hormonal homeostasis seemed to be affected in nrt2 , which displays priming of salicylic acid signaling and concomitant irregular functioning of the jasmonic acid and abscisic acid pathways upon infection .
	manualset3
182016	1	414032	7	NULL	NULL	0	NULL	stress treatments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These stress treatments led to increases in cuticular wax amount per unit area of 32 % to 80 % , due primarily to 29 % to 98 % increases in wax alkanes .
	manualset3
182017	2	414032	7	NULL	NULL	NULL	NULL	cuticular wax amount per unit area	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These stress treatments led to increases in cuticular wax amount per unit area of 32 % to 80 % , due primarily to 29 % to 98 % increases in wax alkanes .
	manualset3
182018	3	414032	7	NULL	NULL	0	NULL	32 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These stress treatments led to increases in cuticular wax amount per unit area of 32 % to 80 % , due primarily to 29 % to 98 % increases in wax alkanes .
	manualset3
182019	4	414032	7	NULL	NULL	0	NULL	80 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These stress treatments led to increases in cuticular wax amount per unit area of 32 % to 80 % , due primarily to 29 % to 98 % increases in wax alkanes .
	manualset3
182020	5	414032	7	NULL	NULL	0	NULL	29 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These stress treatments led to increases in cuticular wax amount per unit area of 32 % to 80 % , due primarily to 29 % to 98 % increases in wax alkanes .
	manualset3
182021	6	414032	7	NULL	NULL	0	NULL	98 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These stress treatments led to increases in cuticular wax amount per unit area of 32 % to 80 % , due primarily to 29 % to 98 % increases in wax alkanes .
	manualset3
182022	7	414032	7	NULL	NULL	0	NULL	wax alkanes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These stress treatments led to increases in cuticular wax amount per unit area of 32 % to 80 % , due primarily to 29 % to 98 % increases in wax alkanes .
	manualset3
182023	1	414033	7	NULL	NULL	0	NULL	strips	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These strips then responded normally to a second addition of platelet activating factor .
	manualset3
182024	2	414033	7	NULL	NULL	0	NULL	second addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These strips then responded normally to a second addition of platelet activating factor .
	manualset3
182025	3	414033	7	NULL	NULL	0	NULL	platelet activating factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These strips then responded normally to a second addition of platelet activating factor .
	manualset3
182026	1	414034	7	NULL	NULL	0	NULL	 structures 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These structures result from the hyperconjugation of the N lone pair to the considered sigma * ( C-H ) orbitals ( TEA-S ) or to the sigma * ( C-C ) and sigma * ( C-H ) orbitals of the CH2 groups ( TEA-AS ) .
	manualset3
182027	2	414034	7	NULL	NULL	0	NULL	hyperconjugation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These structures result from the hyperconjugation of the N lone pair to the considered sigma * ( C-H ) orbitals ( TEA-S ) or to the sigma * ( C-C ) and sigma * ( C-H ) orbitals of the CH2 groups ( TEA-AS ) .
	manualset3
182028	3	414034	7	NULL	NULL	0	NULL	 N lone pair	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	These structures result from the hyperconjugation of the N lone pair to the considered sigma * ( C-H ) orbitals ( TEA-S ) or to the sigma * ( C-C ) and sigma * ( C-H ) orbitals of the CH2 groups ( TEA-AS ) .
	manualset3
182029	4	414034	7	NULL	NULL	NULL	NULL	sigma * ( C-H ) orbitals ( TEA-S )	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These structures result from the hyperconjugation of the N lone pair to the considered sigma * ( C-H ) orbitals ( TEA-S ) or to the sigma * ( C-C ) and sigma * ( C-H ) orbitals of the CH2 groups ( TEA-AS ) .
	manualset3
182031	6	414034	7	NULL	NULL	NULL	NULL	sigma * ( C-C ) orbitals	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These structures result from the hyperconjugation of the N lone pair to the considered sigma * ( C-H ) orbitals ( TEA-S ) or to the sigma * ( C-C ) and sigma * ( C-H ) orbitals of the CH2 groups ( TEA-AS ) .
	manualset3
182032	7	414034	7	NULL	NULL	NULL	NULL	sigma * ( C-H ) orbitals	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These structures result from the hyperconjugation of the N lone pair to the considered sigma * ( C-H ) orbitals ( TEA-S ) or to the sigma * ( C-C ) and sigma * ( C-H ) orbitals of the CH2 groups ( TEA-AS ) .
	manualset3
182033	8	414034	7	NULL	NULL	NULL	NULL	CH2 groups ( TEA-AS )	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These structures result from the hyperconjugation of the N lone pair to the considered sigma * ( C-H ) orbitals ( TEA-S ) or to the sigma * ( C-C ) and sigma * ( C-H ) orbitals of the CH2 groups ( TEA-AS ) .
	manualset3
182034	1	414035	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies also revealed a significant overlap with genes regulated during effector-triggered immunity ( ETI ) .
	manualset3
182035	2	414035	7	NULL	NULL	0	NULL	genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies also revealed a significant overlap with genes regulated during effector-triggered immunity ( ETI ) .
	manualset3
182036	3	414035	7	NULL	NULL	0	NULL	effector-triggered immunity ( ETI )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies also revealed a significant overlap with genes regulated during effector-triggered immunity ( ETI ) .
	manualset3
182037	1	414036	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies establish ezetimibe as an effective lipid-lowering agent , which will likely be useful in the management of a broad range of patients with hypercholesterolemia .
	manualset3
182038	2	414036	7	NULL	NULL	0	NULL	ezetimibe	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies establish ezetimibe as an effective lipid-lowering agent , which will likely be useful in the management of a broad range of patients with hypercholesterolemia .
	manualset3
182039	3	414036	7	NULL	NULL	0	NULL	effective lipid-lowering agent	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies establish ezetimibe as an effective lipid-lowering agent , which will likely be useful in the management of a broad range of patients with hypercholesterolemia .
	manualset3
182040	4	414036	7	NULL	NULL	0	NULL	useful	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies establish ezetimibe as an effective lipid-lowering agent , which will likely be useful in the management of a broad range of patients with hypercholesterolemia .
	manualset3
182041	5	414036	7	NULL	NULL	0	NULL	management 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies establish ezetimibe as an effective lipid-lowering agent , which will likely be useful in the management of a broad range of patients with hypercholesterolemia .
	manualset3
182042	6	414036	7	NULL	NULL	0	NULL	broad range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies establish ezetimibe as an effective lipid-lowering agent , which will likely be useful in the management of a broad range of patients with hypercholesterolemia .
	manualset3
182043	7	414036	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies establish ezetimibe as an effective lipid-lowering agent , which will likely be useful in the management of a broad range of patients with hypercholesterolemia .
	manualset3
182044	8	414036	7	NULL	NULL	0	NULL	hypercholesterolemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies establish ezetimibe as an effective lipid-lowering agent , which will likely be useful in the management of a broad range of patients with hypercholesterolemia .
	manualset3
182045	1	414037	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies have suggested that the use of HME filters may be effective in preserving body temperature and airway humidity while decreasing fluid build-up in the breathing system and therefore reducing breathing system contamination .
	manualset3
182046	2	414037	7	NULL	NULL	0	NULL	HME filters	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies have suggested that the use of HME filters may be effective in preserving body temperature and airway humidity while decreasing fluid build-up in the breathing system and therefore reducing breathing system contamination .
	manualset3
182047	3	414037	7	NULL	NULL	0	NULL	preserving	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies have suggested that the use of HME filters may be effective in preserving body temperature and airway humidity while decreasing fluid build-up in the breathing system and therefore reducing breathing system contamination .
	manualset3
182048	4	414037	7	NULL	NULL	0	NULL	body temperature	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies have suggested that the use of HME filters may be effective in preserving body temperature and airway humidity while decreasing fluid build-up in the breathing system and therefore reducing breathing system contamination .
	manualset3
182049	5	414037	7	NULL	NULL	0	NULL	airway humidity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies have suggested that the use of HME filters may be effective in preserving body temperature and airway humidity while decreasing fluid build-up in the breathing system and therefore reducing breathing system contamination .
	manualset3
182050	6	414037	7	NULL	NULL	0	NULL	decreasing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies have suggested that the use of HME filters may be effective in preserving body temperature and airway humidity while decreasing fluid build-up in the breathing system and therefore reducing breathing system contamination .
	manualset3
182051	7	414037	7	NULL	NULL	0	NULL	fluid build-up	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies have suggested that the use of HME filters may be effective in preserving body temperature and airway humidity while decreasing fluid build-up in the breathing system and therefore reducing breathing system contamination .
	manualset3
182052	8	414037	7	NULL	NULL	0	NULL	 breathing system 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies have suggested that the use of HME filters may be effective in preserving body temperature and airway humidity while decreasing fluid build-up in the breathing system and therefore reducing breathing system contamination .
	manualset3
182053	9	414037	7	NULL	NULL	0	NULL	 reducing 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies have suggested that the use of HME filters may be effective in preserving body temperature and airway humidity while decreasing fluid build-up in the breathing system and therefore reducing breathing system contamination .
	manualset3
182054	10	414037	7	NULL	NULL	0	NULL	breathing system contamination	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies have suggested that the use of HME filters may be effective in preserving body temperature and airway humidity while decreasing fluid build-up in the breathing system and therefore reducing breathing system contamination .
	manualset3
182066	1	414039	7	NULL	NULL	0	NULL	 families	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , in families with longevity members , alleles and haplotypes positively associated with autoimmunity were not observed .
	manualset3
182067	2	414039	7	NULL	NULL	0	NULL	longevity members	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , in families with longevity members , alleles and haplotypes positively associated with autoimmunity were not observed .
	manualset3
182068	3	414039	7	NULL	NULL	0	NULL	alleles 	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , in families with longevity members , alleles and haplotypes positively associated with autoimmunity were not observed .
	manualset3
182069	4	414039	7	NULL	NULL	0	NULL	haplotypes 	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , in families with longevity members , alleles and haplotypes positively associated with autoimmunity were not observed .
	manualset3
182070	5	414039	7	NULL	NULL	0	NULL	autoimmunity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , in families with longevity members , alleles and haplotypes positively associated with autoimmunity were not observed .
	manualset3
182071	1	414040	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies indicate that adhesion and migration of T lymphocytes across the cerebral endothelial barrier are distinct processes that depend upon the activation state of EC and are controlled by diverse receptor-ligand interactions .
	manualset3
182072	2	414040	7	NULL	NULL	0	NULL	adhesion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies indicate that adhesion and migration of T lymphocytes across the cerebral endothelial barrier are distinct processes that depend upon the activation state of EC and are controlled by diverse receptor-ligand interactions .
	manualset3
182073	3	414040	7	NULL	NULL	0	NULL	migration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies indicate that adhesion and migration of T lymphocytes across the cerebral endothelial barrier are distinct processes that depend upon the activation state of EC and are controlled by diverse receptor-ligand interactions .
	manualset3
182074	4	414040	7	NULL	NULL	0	NULL	T lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies indicate that adhesion and migration of T lymphocytes across the cerebral endothelial barrier are distinct processes that depend upon the activation state of EC and are controlled by diverse receptor-ligand interactions .
	manualset3
182075	5	414040	7	NULL	NULL	0	NULL	cerebral endothelial barrier	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies indicate that adhesion and migration of T lymphocytes across the cerebral endothelial barrier are distinct processes that depend upon the activation state of EC and are controlled by diverse receptor-ligand interactions .
	manualset3
182076	6	414040	7	NULL	NULL	0	NULL	processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies indicate that adhesion and migration of T lymphocytes across the cerebral endothelial barrier are distinct processes that depend upon the activation state of EC and are controlled by diverse receptor-ligand interactions .
	manualset3
182077	7	414040	7	NULL	NULL	0	NULL	activation state	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies indicate that adhesion and migration of T lymphocytes across the cerebral endothelial barrier are distinct processes that depend upon the activation state of EC and are controlled by diverse receptor-ligand interactions .
	manualset3
182078	8	414040	7	NULL	NULL	0	NULL	EC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies indicate that adhesion and migration of T lymphocytes across the cerebral endothelial barrier are distinct processes that depend upon the activation state of EC and are controlled by diverse receptor-ligand interactions .
	manualset3
182079	9	414040	7	NULL	NULL	0	NULL	receptor-ligand interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies indicate that adhesion and migration of T lymphocytes across the cerebral endothelial barrier are distinct processes that depend upon the activation state of EC and are controlled by diverse receptor-ligand interactions .
	manualset3
182257	1	414041	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies indicate that lymphocyte adhesion to central nervous system ( CNS ) vascular EC is largely dependent on LFA-1 but not through its interaction with ICAM-1 .
	manualset3
182258	2	414041	7	NULL	NULL	0	NULL	lymphocyte adhesion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies indicate that lymphocyte adhesion to central nervous system ( CNS ) vascular EC is largely dependent on LFA-1 but not through its interaction with ICAM-1 .
	manualset3
182259	3	414041	7	NULL	NULL	NULL	NULL	central nervous system ( CNS ) vascular EC	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These studies indicate that lymphocyte adhesion to central nervous system ( CNS ) vascular EC is largely dependent on LFA-1 but not through its interaction with ICAM-1 .
	manualset3
182260	4	414041	7	NULL	NULL	NULL	NULL	LFA-1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These studies indicate that lymphocyte adhesion to central nervous system ( CNS ) vascular EC is largely dependent on LFA-1 but not through its interaction with ICAM-1 .
	manualset3
182261	5	414041	7	NULL	NULL	0	NULL	 interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies indicate that lymphocyte adhesion to central nervous system ( CNS ) vascular EC is largely dependent on LFA-1 but not through its interaction with ICAM-1 .
	manualset3
182262	6	414041	7	NULL	NULL	0	NULL	ICAM-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies indicate that lymphocyte adhesion to central nervous system ( CNS ) vascular EC is largely dependent on LFA-1 but not through its interaction with ICAM-1 .
	manualset3
182263	1	414042	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies indicate that the BPH stroma is not only a preferential tissue for 5 alpha-reductase activity and DHT enrichment but also for nuclear estradiol accumulation .
	manualset3
182264	2	414042	7	NULL	NULL	0	NULL	BPH stroma	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies indicate that the BPH stroma is not only a preferential tissue for 5 alpha-reductase activity and DHT enrichment but also for nuclear estradiol accumulation .
	manualset3
182265	3	414042	7	NULL	NULL	0	NULL	tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies indicate that the BPH stroma is not only a preferential tissue for 5 alpha-reductase activity and DHT enrichment but also for nuclear estradiol accumulation .
	manualset3
182266	4	414042	7	NULL	NULL	0	NULL	5 alpha-reductase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies indicate that the BPH stroma is not only a preferential tissue for 5 alpha-reductase activity and DHT enrichment but also for nuclear estradiol accumulation .
	manualset3
182267	5	414042	7	NULL	NULL	0	NULL	DHT enrichment 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies indicate that the BPH stroma is not only a preferential tissue for 5 alpha-reductase activity and DHT enrichment but also for nuclear estradiol accumulation .
	manualset3
182269	6	414042	7	NULL	NULL	0	NULL	nuclear estradiol accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies indicate that the BPH stroma is not only a preferential tissue for 5 alpha-reductase activity and DHT enrichment but also for nuclear estradiol accumulation .
	manualset3
182281	1	414043	7	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies provide a mechanism by which Apaf-1 promotes autoactivation of pro-casp9 through Apaf-1 self-association , a process that is negatively regulated by the WD-40 repeats .
	manualset3
182283	2	414043	7	NULL	NULL	0	NULL	mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies provide a mechanism by which Apaf-1 promotes autoactivation of pro-casp9 through Apaf-1 self-association , a process that is negatively regulated by the WD-40 repeats .
	manualset3
182286	3	414043	7	NULL	NULL	0	NULL	Apaf-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies provide a mechanism by which Apaf-1 promotes autoactivation of pro-casp9 through Apaf-1 self-association , a process that is negatively regulated by the WD-40 repeats .
	manualset3
182288	4	414043	7	NULL	NULL	0	NULL	autoactivation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies provide a mechanism by which Apaf-1 promotes autoactivation of pro-casp9 through Apaf-1 self-association , a process that is negatively regulated by the WD-40 repeats .
	manualset3
182291	5	414043	7	NULL	NULL	0	NULL	pro-casp9	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies provide a mechanism by which Apaf-1 promotes autoactivation of pro-casp9 through Apaf-1 self-association , a process that is negatively regulated by the WD-40 repeats .
	manualset3
182293	6	414043	7	NULL	NULL	0	NULL	Apaf-1 self-association	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies provide a mechanism by which Apaf-1 promotes autoactivation of pro-casp9 through Apaf-1 self-association , a process that is negatively regulated by the WD-40 repeats .
	manualset3
182296	7	414043	7	NULL	NULL	0	NULL	process	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies provide a mechanism by which Apaf-1 promotes autoactivation of pro-casp9 through Apaf-1 self-association , a process that is negatively regulated by the WD-40 repeats .
	manualset3
182298	8	414043	7	NULL	NULL	0	NULL	WD-40 repeats	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies provide a mechanism by which Apaf-1 promotes autoactivation of pro-casp9 through Apaf-1 self-association , a process that is negatively regulated by the WD-40 repeats .
	manualset3
182300	1	414044	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies showed that production of CART peptides by bacterial expression is a viable alternative to current methods .
	manualset3
182301	2	414044	7	NULL	NULL	0	NULL	production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies showed that production of CART peptides by bacterial expression is a viable alternative to current methods .
	manualset3
182303	3	414044	7	NULL	NULL	0	NULL	CART peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies showed that production of CART peptides by bacterial expression is a viable alternative to current methods .
	manualset3
182305	4	414044	7	NULL	NULL	0	NULL	bacterial expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies showed that production of CART peptides by bacterial expression is a viable alternative to current methods .
	manualset3
182307	5	414044	7	NULL	NULL	0	NULL	 viable alternative method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies showed that production of CART peptides by bacterial expression is a viable alternative to current methods .
	manualset3
182309	6	414044	7	NULL	NULL	0	NULL	current methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies showed that production of CART peptides by bacterial expression is a viable alternative to current methods .
	manualset3
182351	1	414045	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that , in addition to its ability to inhibit tumor vascularization , angiostatin 2epsilon may also directly block tumor metastasis .
	manualset3
182352	2	414045	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that , in addition to its ability to inhibit tumor vascularization , angiostatin 2epsilon may also directly block tumor metastasis .
	manualset3
182353	3	414045	7	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that , in addition to its ability to inhibit tumor vascularization , angiostatin 2epsilon may also directly block tumor metastasis .
	manualset3
182354	4	414045	7	NULL	NULL	0	NULL	tumor vascularization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that , in addition to its ability to inhibit tumor vascularization , angiostatin 2epsilon may also directly block tumor metastasis .
	manualset3
182355	5	414045	7	NULL	NULL	0	NULL	angiostatin 2epsilon 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that , in addition to its ability to inhibit tumor vascularization , angiostatin 2epsilon may also directly block tumor metastasis .
	manualset3
182356	6	414045	7	NULL	NULL	0	NULL	tumor metastasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that , in addition to its ability to inhibit tumor vascularization , angiostatin 2epsilon may also directly block tumor metastasis .
	manualset3
182357	1	414046	7	NULL	NULL	0	NULL	 studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that , in lower concentrations , TMB-8 inhibits the mobilization of iCa2 + , which is important for the interaction of Gs with the catalytic unit of adenylyl cyclase and the initial increase in AVP-stimulated Pf .
	manualset3
182358	2	414046	7	NULL	NULL	0	NULL	lower concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that , in lower concentrations , TMB-8 inhibits the mobilization of iCa2 + , which is important for the interaction of Gs with the catalytic unit of adenylyl cyclase and the initial increase in AVP-stimulated Pf .
	manualset3
182359	3	414046	7	NULL	NULL	0	NULL	 TMB-8 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that , in lower concentrations , TMB-8 inhibits the mobilization of iCa2 + , which is important for the interaction of Gs with the catalytic unit of adenylyl cyclase and the initial increase in AVP-stimulated Pf .
	manualset3
182360	4	414046	7	NULL	NULL	0	NULL	mobilization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that , in lower concentrations , TMB-8 inhibits the mobilization of iCa2 + , which is important for the interaction of Gs with the catalytic unit of adenylyl cyclase and the initial increase in AVP-stimulated Pf .
	manualset3
182361	5	414046	7	NULL	NULL	0	NULL	iCa2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that , in lower concentrations , TMB-8 inhibits the mobilization of iCa2 + , which is important for the interaction of Gs with the catalytic unit of adenylyl cyclase and the initial increase in AVP-stimulated Pf .
	manualset3
182362	6	414046	7	NULL	NULL	0	NULL	interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that , in lower concentrations , TMB-8 inhibits the mobilization of iCa2 + , which is important for the interaction of Gs with the catalytic unit of adenylyl cyclase and the initial increase in AVP-stimulated Pf .
	manualset3
182363	7	414046	7	NULL	NULL	0	NULL	Gs	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that , in lower concentrations , TMB-8 inhibits the mobilization of iCa2 + , which is important for the interaction of Gs with the catalytic unit of adenylyl cyclase and the initial increase in AVP-stimulated Pf .
	manualset3
182364	8	414046	7	NULL	NULL	0	NULL	catalytic unit	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that , in lower concentrations , TMB-8 inhibits the mobilization of iCa2 + , which is important for the interaction of Gs with the catalytic unit of adenylyl cyclase and the initial increase in AVP-stimulated Pf .
	manualset3
182365	9	414046	7	NULL	NULL	0	NULL	adenylyl cyclase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that , in lower concentrations , TMB-8 inhibits the mobilization of iCa2 + , which is important for the interaction of Gs with the catalytic unit of adenylyl cyclase and the initial increase in AVP-stimulated Pf .
	manualset3
182366	10	414046	7	NULL	NULL	0	NULL	initial increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that , in lower concentrations , TMB-8 inhibits the mobilization of iCa2 + , which is important for the interaction of Gs with the catalytic unit of adenylyl cyclase and the initial increase in AVP-stimulated Pf .
	manualset3
182367	11	414046	7	NULL	NULL	0	NULL	AVP-stimulated Pf	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that , in lower concentrations , TMB-8 inhibits the mobilization of iCa2 + , which is important for the interaction of Gs with the catalytic unit of adenylyl cyclase and the initial increase in AVP-stimulated Pf .
	manualset3
182406	1	414047	7	NULL	NULL	0	NULL	 studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that HER-3 could be used as a biomarker to select patients who are most likely to respond to erlotinib therapy .
	manualset3
182407	2	414047	7	NULL	NULL	0	NULL	HER-3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that HER-3 could be used as a biomarker to select patients who are most likely to respond to erlotinib therapy .
	manualset3
182413	3	414047	7	NULL	NULL	0	NULL	biomarker	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that HER-3 could be used as a biomarker to select patients who are most likely to respond to erlotinib therapy .
	manualset3
182414	4	414047	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that HER-3 could be used as a biomarker to select patients who are most likely to respond to erlotinib therapy .
	manualset3
182415	5	414047	7	NULL	NULL	0	NULL	erlotinib therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that HER-3 could be used as a biomarker to select patients who are most likely to respond to erlotinib therapy .
	manualset3
182418	1	414048	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that amelioration of hypokalemia attenuates mineralocorticoid-induced sodium retention .
	manualset3
182420	2	414048	7	NULL	NULL	0	NULL	amelioration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that amelioration of hypokalemia attenuates mineralocorticoid-induced sodium retention .
	manualset3
182423	3	414048	7	NULL	NULL	0	NULL	hypokalemia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that amelioration of hypokalemia attenuates mineralocorticoid-induced sodium retention .
	manualset3
182424	4	414048	7	NULL	NULL	0	NULL	mineralocorticoid-induced sodium retention	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that amelioration of hypokalemia attenuates mineralocorticoid-induced sodium retention .
	manualset3
182425	1	414049	7	NULL	NULL	0	NULL	 studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that the generation of SAA after endotoxin administration does not involve complement activation or intravascular proteolytic activity , whereas the liberation of a specific peptic-like cleavage product of albumin appears to be the consequence of an acid protease .
	manualset3
182433	2	414049	7	NULL	NULL	0	NULL	 generation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that the generation of SAA after endotoxin administration does not involve complement activation or intravascular proteolytic activity , whereas the liberation of a specific peptic-like cleavage product of albumin appears to be the consequence of an acid protease .
	manualset3
182436	3	414049	7	NULL	NULL	0	NULL	SAA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that the generation of SAA after endotoxin administration does not involve complement activation or intravascular proteolytic activity , whereas the liberation of a specific peptic-like cleavage product of albumin appears to be the consequence of an acid protease .
	manualset3
182437	4	414049	7	NULL	NULL	0	NULL	endotoxin administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that the generation of SAA after endotoxin administration does not involve complement activation or intravascular proteolytic activity , whereas the liberation of a specific peptic-like cleavage product of albumin appears to be the consequence of an acid protease .
	manualset3
182438	5	414049	7	NULL	NULL	0	NULL	complement activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that the generation of SAA after endotoxin administration does not involve complement activation or intravascular proteolytic activity , whereas the liberation of a specific peptic-like cleavage product of albumin appears to be the consequence of an acid protease .
	manualset3
182440	6	414049	7	NULL	NULL	0	NULL	intravascular proteolytic activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that the generation of SAA after endotoxin administration does not involve complement activation or intravascular proteolytic activity , whereas the liberation of a specific peptic-like cleavage product of albumin appears to be the consequence of an acid protease .
	manualset3
182444	7	414049	7	NULL	NULL	0	NULL	liberation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that the generation of SAA after endotoxin administration does not involve complement activation or intravascular proteolytic activity , whereas the liberation of a specific peptic-like cleavage product of albumin appears to be the consequence of an acid protease .
	manualset3
182445	8	414049	7	NULL	NULL	0	NULL	 peptic-like cleavage product 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that the generation of SAA after endotoxin administration does not involve complement activation or intravascular proteolytic activity , whereas the liberation of a specific peptic-like cleavage product of albumin appears to be the consequence of an acid protease .
	manualset3
182446	9	414049	7	NULL	NULL	0	NULL	albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that the generation of SAA after endotoxin administration does not involve complement activation or intravascular proteolytic activity , whereas the liberation of a specific peptic-like cleavage product of albumin appears to be the consequence of an acid protease .
	manualset3
182449	10	414049	7	NULL	NULL	0	NULL	acid protease	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that the generation of SAA after endotoxin administration does not involve complement activation or intravascular proteolytic activity , whereas the liberation of a specific peptic-like cleavage product of albumin appears to be the consequence of an acid protease .
	manualset3
182456	1	414050	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that the impaired response of nephrotic lymphocytes to phytohaemagglutinin is a secondary consequence of the nephrotic state , probably attributable , at least in part , to increased prostaglandin production in the nephrotic syndrome .
	manualset3
182459	2	414050	7	NULL	NULL	0	NULL	impaired response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that the impaired response of nephrotic lymphocytes to phytohaemagglutinin is a secondary consequence of the nephrotic state , probably attributable , at least in part , to increased prostaglandin production in the nephrotic syndrome .
	manualset3
182461	3	414050	7	NULL	NULL	0	NULL	nephrotic lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that the impaired response of nephrotic lymphocytes to phytohaemagglutinin is a secondary consequence of the nephrotic state , probably attributable , at least in part , to increased prostaglandin production in the nephrotic syndrome .
	manualset3
182464	4	414050	7	NULL	NULL	0	NULL	 phytohaemagglutinin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that the impaired response of nephrotic lymphocytes to phytohaemagglutinin is a secondary consequence of the nephrotic state , probably attributable , at least in part , to increased prostaglandin production in the nephrotic syndrome .
	manualset3
182469	5	414050	7	NULL	NULL	0	NULL	secondary consequence	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that the impaired response of nephrotic lymphocytes to phytohaemagglutinin is a secondary consequence of the nephrotic state , probably attributable , at least in part , to increased prostaglandin production in the nephrotic syndrome .
	manualset3
182472	6	414050	7	NULL	NULL	0	NULL	nephrotic state	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that the impaired response of nephrotic lymphocytes to phytohaemagglutinin is a secondary consequence of the nephrotic state , probably attributable , at least in part , to increased prostaglandin production in the nephrotic syndrome .
	manualset3
182473	7	414050	7	NULL	NULL	0	NULL	increased prostaglandin production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that the impaired response of nephrotic lymphocytes to phytohaemagglutinin is a secondary consequence of the nephrotic state , probably attributable , at least in part , to increased prostaglandin production in the nephrotic syndrome .
	manualset3
182474	8	414050	7	NULL	NULL	0	NULL	nephrotic syndrome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies suggest that the impaired response of nephrotic lymphocytes to phytohaemagglutinin is a secondary consequence of the nephrotic state , probably attributable , at least in part , to increased prostaglandin production in the nephrotic syndrome .
	manualset3
182489	1	414051	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies therefore show that endothelialization of these polyurethane surfaces is feasible .
	manualset3
182490	2	414051	7	NULL	NULL	0	NULL	endothelialization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies therefore show that endothelialization of these polyurethane surfaces is feasible .
	manualset3
182491	3	414051	7	NULL	NULL	0	NULL	polyurethane surfaces	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These studies therefore show that endothelialization of these polyurethane surfaces is feasible .
	manualset3
182492	1	414052	7	NULL	NULL	0	NULL	 subsets	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These subsets regulate the nature of a T cell-mediated immune response .
	manualset3
182493	2	414052	7	NULL	NULL	0	NULL	nature 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These subsets regulate the nature of a T cell-mediated immune response .
	manualset3
182494	3	414052	7	NULL	NULL	0	NULL	T cell-mediated immune response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These subsets regulate the nature of a T cell-mediated immune response .
	manualset3
182495	1	414053	7	NULL	NULL	NULL	NULL	targets 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These targets included the tumor-suppressive genes large tumor suppressor 2 ( LATS2 ) and PP2A regulatory subunit B alpha isoform ( PPP2R2A ) , and expression of each was augmented by miR-31 knockdown .
	manualset3
182496	2	414053	7	NULL	NULL	0	NULL	tumor-suppressive genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These targets included the tumor-suppressive genes large tumor suppressor 2 ( LATS2 ) and PP2A regulatory subunit B alpha isoform ( PPP2R2A ) , and expression of each was augmented by miR-31 knockdown .
	manualset3
182497	3	414053	7	NULL	NULL	0	NULL	large tumor suppressor 2 ( LATS2 ) 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	These targets included the tumor-suppressive genes large tumor suppressor 2 ( LATS2 ) and PP2A regulatory subunit B alpha isoform ( PPP2R2A ) , and expression of each was augmented by miR-31 knockdown .
	manualset3
182498	4	414053	7	NULL	NULL	0	NULL	PP2A regulatory subunit B alpha isoform ( PPP2R2A )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	These targets included the tumor-suppressive genes large tumor suppressor 2 ( LATS2 ) and PP2A regulatory subunit B alpha isoform ( PPP2R2A ) , and expression of each was augmented by miR-31 knockdown .
	manualset3
182499	5	414053	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These targets included the tumor-suppressive genes large tumor suppressor 2 ( LATS2 ) and PP2A regulatory subunit B alpha isoform ( PPP2R2A ) , and expression of each was augmented by miR-31 knockdown .
	manualset3
182500	6	414053	7	NULL	NULL	0	NULL	miR-31 knockdown	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These targets included the tumor-suppressive genes large tumor suppressor 2 ( LATS2 ) and PP2A regulatory subunit B alpha isoform ( PPP2R2A ) , and expression of each was augmented by miR-31 knockdown .
	manualset3
182501	1	414054	7	NULL	NULL	0	NULL	 techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These techniques , in concert with new methods of microscopy , isolation of new metabolic groups , and the study of new ecosystems , suggest that there is much that will be learned about the microbiology of sedimentary environments in the coming years .
	manualset3
182502	2	414054	7	NULL	NULL	0	NULL	new methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These techniques , in concert with new methods of microscopy , isolation of new metabolic groups , and the study of new ecosystems , suggest that there is much that will be learned about the microbiology of sedimentary environments in the coming years .
	manualset3
182503	3	414054	7	NULL	NULL	0	NULL	microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These techniques , in concert with new methods of microscopy , isolation of new metabolic groups , and the study of new ecosystems , suggest that there is much that will be learned about the microbiology of sedimentary environments in the coming years .
	manualset3
182504	4	414054	7	NULL	NULL	0	NULL	 isolation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These techniques , in concert with new methods of microscopy , isolation of new metabolic groups , and the study of new ecosystems , suggest that there is much that will be learned about the microbiology of sedimentary environments in the coming years .
	manualset3
182505	5	414054	7	NULL	NULL	0	NULL	new metabolic groups 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These techniques , in concert with new methods of microscopy , isolation of new metabolic groups , and the study of new ecosystems , suggest that there is much that will be learned about the microbiology of sedimentary environments in the coming years .
	manualset3
182506	6	414054	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These techniques , in concert with new methods of microscopy , isolation of new metabolic groups , and the study of new ecosystems , suggest that there is much that will be learned about the microbiology of sedimentary environments in the coming years .
	manualset3
182507	7	414054	7	NULL	NULL	0	NULL	new ecosystems	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These techniques , in concert with new methods of microscopy , isolation of new metabolic groups , and the study of new ecosystems , suggest that there is much that will be learned about the microbiology of sedimentary environments in the coming years .
	manualset3
182508	8	414054	7	NULL	NULL	0	NULL	microbiology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These techniques , in concert with new methods of microscopy , isolation of new metabolic groups , and the study of new ecosystems , suggest that there is much that will be learned about the microbiology of sedimentary environments in the coming years .
	manualset3
182509	9	414054	7	NULL	NULL	0	NULL	sedimentary environments	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These techniques , in concert with new methods of microscopy , isolation of new metabolic groups , and the study of new ecosystems , suggest that there is much that will be learned about the microbiology of sedimentary environments in the coming years .
	manualset3
182510	10	414054	7	NULL	NULL	0	NULL	years	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	These techniques , in concert with new methods of microscopy , isolation of new metabolic groups , and the study of new ecosystems , suggest that there is much that will be learned about the microbiology of sedimentary environments in the coming years .
	manualset3
182511	1	414055	7	NULL	NULL	NULL	NULL	tools	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These tools include clinical decision support , vaccination coverage reports , interoperability with electronic health record systems , vaccine inventory management , and the ability to generate reminder and recall messages .
	manualset3
182512	2	414055	7	NULL	NULL	0	NULL	clinical decision support	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These tools include clinical decision support , vaccination coverage reports , interoperability with electronic health record systems , vaccine inventory management , and the ability to generate reminder and recall messages .
	manualset3
182513	3	414055	7	NULL	NULL	0	NULL	vaccination coverage reports	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These tools include clinical decision support , vaccination coverage reports , interoperability with electronic health record systems , vaccine inventory management , and the ability to generate reminder and recall messages .
	manualset3
182514	4	414055	7	NULL	NULL	0	NULL	interoperability with electronic health record systems	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	These tools include clinical decision support , vaccination coverage reports , interoperability with electronic health record systems , vaccine inventory management , and the ability to generate reminder and recall messages .
	manualset3
182515	5	414055	7	NULL	NULL	0	NULL	vaccine inventory management	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These tools include clinical decision support , vaccination coverage reports , interoperability with electronic health record systems , vaccine inventory management , and the ability to generate reminder and recall messages .
	manualset3
182516	6	414055	7	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These tools include clinical decision support , vaccination coverage reports , interoperability with electronic health record systems , vaccine inventory management , and the ability to generate reminder and recall messages .
	manualset3
182517	7	414055	7	NULL	NULL	0	NULL	reminder messages	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These tools include clinical decision support , vaccination coverage reports , interoperability with electronic health record systems , vaccine inventory management , and the ability to generate reminder and recall messages .
	manualset3
182518	8	414055	7	NULL	NULL	0	NULL	 recall messages	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These tools include clinical decision support , vaccination coverage reports , interoperability with electronic health record systems , vaccine inventory management , and the ability to generate reminder and recall messages .
	manualset3
182519	1	414056	7	NULL	NULL	0	NULL	toxins	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	These toxins are - helical peptides with a formyl group at the N terminus , and they activate neutrophils through formyl peptide receptor 2 ( FPR2 ) , a function closely correlated to the capacity of staphylococcal species to cause invasive infections .
	manualset3
182520	2	414056	7	NULL	NULL	0	NULL	helical peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	These toxins are - helical peptides with a formyl group at the N terminus , and they activate neutrophils through formyl peptide receptor 2 ( FPR2 ) , a function closely correlated to the capacity of staphylococcal species to cause invasive infections .
	manualset3
182521	3	414056	7	NULL	NULL	NULL	NULL	formyl group 	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These toxins are - helical peptides with a formyl group at the N terminus , and they activate neutrophils through formyl peptide receptor 2 ( FPR2 ) , a function closely correlated to the capacity of staphylococcal species to cause invasive infections .
	manualset3
182522	4	414056	7	NULL	NULL	0	NULL	N terminus	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These toxins are - helical peptides with a formyl group at the N terminus , and they activate neutrophils through formyl peptide receptor 2 ( FPR2 ) , a function closely correlated to the capacity of staphylococcal species to cause invasive infections .
	manualset3
182523	5	414056	7	NULL	NULL	0	NULL	neutrophils	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These toxins are - helical peptides with a formyl group at the N terminus , and they activate neutrophils through formyl peptide receptor 2 ( FPR2 ) , a function closely correlated to the capacity of staphylococcal species to cause invasive infections .
	manualset3
182524	6	414056	7	NULL	NULL	0	NULL	formyl peptide receptor 2 ( FPR2 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These toxins are - helical peptides with a formyl group at the N terminus , and they activate neutrophils through formyl peptide receptor 2 ( FPR2 ) , a function closely correlated to the capacity of staphylococcal species to cause invasive infections .
	manualset3
182525	7	414056	7	NULL	NULL	0	NULL	function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These toxins are - helical peptides with a formyl group at the N terminus , and they activate neutrophils through formyl peptide receptor 2 ( FPR2 ) , a function closely correlated to the capacity of staphylococcal species to cause invasive infections .
	manualset3
182526	8	414056	7	NULL	NULL	0	NULL	capacity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These toxins are - helical peptides with a formyl group at the N terminus , and they activate neutrophils through formyl peptide receptor 2 ( FPR2 ) , a function closely correlated to the capacity of staphylococcal species to cause invasive infections .
	manualset3
182527	9	414056	7	NULL	NULL	0	NULL	staphylococcal species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These toxins are - helical peptides with a formyl group at the N terminus , and they activate neutrophils through formyl peptide receptor 2 ( FPR2 ) , a function closely correlated to the capacity of staphylococcal species to cause invasive infections .
	manualset3
182528	10	414056	7	NULL	NULL	NULL	NULL	invasive infections	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These toxins are - helical peptides with a formyl group at the N terminus , and they activate neutrophils through formyl peptide receptor 2 ( FPR2 ) , a function closely correlated to the capacity of staphylococcal species to cause invasive infections .
	manualset3
182529	1	414057	7	NULL	NULL	0	NULL	traits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These traits were characterized by three parameters : average phototactic ( locomotor ) activity , normalized variance of activity and proportion of inactive flies .
	manualset3
182530	2	414057	7	NULL	NULL	0	NULL	three parameters	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These traits were characterized by three parameters : average phototactic ( locomotor ) activity , normalized variance of activity and proportion of inactive flies .
	manualset3
182531	3	414057	7	NULL	NULL	0	NULL	average phototactic ( locomotor ) activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These traits were characterized by three parameters : average phototactic ( locomotor ) activity , normalized variance of activity and proportion of inactive flies .
	manualset3
182532	4	414057	7	NULL	NULL	0	NULL	normalized variance of activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These traits were characterized by three parameters : average phototactic ( locomotor ) activity , normalized variance of activity and proportion of inactive flies .
	manualset3
182533	5	414057	7	NULL	NULL	0	NULL	proportion	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These traits were characterized by three parameters : average phototactic ( locomotor ) activity , normalized variance of activity and proportion of inactive flies .
	manualset3
182534	6	414057	7	NULL	NULL	0	NULL	inactive flies	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These traits were characterized by three parameters : average phototactic ( locomotor ) activity , normalized variance of activity and proportion of inactive flies .
	manualset3
182535	1	414058	7	NULL	NULL	0	NULL	transgenic models	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These transgenic models will be a valuable platform in exploring the mechanism of fibrogenic pancreatic diseases which are induced by Hh signaling activation .
	manualset3
182536	2	414058	7	NULL	NULL	0	NULL	valuable platform	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These transgenic models will be a valuable platform in exploring the mechanism of fibrogenic pancreatic diseases which are induced by Hh signaling activation .
	manualset3
182537	3	414058	7	NULL	NULL	0	NULL	mechanism 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These transgenic models will be a valuable platform in exploring the mechanism of fibrogenic pancreatic diseases which are induced by Hh signaling activation .
	manualset3
182538	4	414058	7	NULL	NULL	0	NULL	fibrogenic pancreatic diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These transgenic models will be a valuable platform in exploring the mechanism of fibrogenic pancreatic diseases which are induced by Hh signaling activation .
	manualset3
182539	5	414058	7	NULL	NULL	0	NULL	Hh signaling activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These transgenic models will be a valuable platform in exploring the mechanism of fibrogenic pancreatic diseases which are induced by Hh signaling activation .
	manualset3
182540	1	414059	7	NULL	NULL	0	NULL	levels of E-2	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , levels of E-2 , 3 - Q-4-S-Alb correlated significantly with those of E-3 , 4 - Q-2-S-Alb ( correlation coefficient r = 0.684-0 .850 , p & lt ; 0.05 ) .
	manualset3
182541	2	414059	7	NULL	NULL	NULL	NULL	levels of E-3- Q-4-S-Alb	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Additionally , levels of E-2 , 3 - Q-4-S-Alb correlated significantly with those of E-3 , 4 - Q-2-S-Alb ( correlation coefficient r = 0.684-0 .850 , p & lt ; 0.05 ) .
	manualset3
182542	3	414059	7	NULL	NULL	0	NULL	E-3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , levels of E-2 , 3 - Q-4-S-Alb correlated significantly with those of E-3 , 4 - Q-2-S-Alb ( correlation coefficient r = 0.684-0 .850 , p & lt ; 0.05 ) .
	manualset3
182543	4	414059	7	NULL	NULL	0	NULL	E-4 - Q-2-S-Alb	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , levels of E-2 , 3 - Q-4-S-Alb correlated significantly with those of E-3 , 4 - Q-2-S-Alb ( correlation coefficient r = 0.684-0 .850 , p & lt ; 0.05 ) .
	manualset3
182544	5	414059	7	NULL	NULL	0	NULL	correlation coefficient	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , levels of E-2 , 3 - Q-4-S-Alb correlated significantly with those of E-3 , 4 - Q-2-S-Alb ( correlation coefficient r = 0.684-0 .850 , p & lt ; 0.05 ) .
	manualset3
182545	6	414059	7	NULL	NULL	0	NULL	 r = 0.684-0 .850	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , levels of E-2 , 3 - Q-4-S-Alb correlated significantly with those of E-3 , 4 - Q-2-S-Alb ( correlation coefficient r = 0.684-0 .850 , p & lt ; 0.05 ) .
	manualset3
182546	7	414059	7	NULL	NULL	0	NULL	p & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , levels of E-2 , 3 - Q-4-S-Alb correlated significantly with those of E-3 , 4 - Q-2-S-Alb ( correlation coefficient r = 0.684-0 .850 , p & lt ; 0.05 ) .
	manualset3
182547	1	414060	7	NULL	NULL	0	NULL	 treatments	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These treatments , therefore , increase the water wetting index .
	manualset3
182548	2	414060	7	NULL	NULL	0	NULL	water wetting index	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These treatments , therefore , increase the water wetting index .
	manualset3
182549	1	414061	7	NULL	NULL	0	NULL	trends	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These trends with age were also expressed as annual rates of change : ABV/TV ( -0.52 % / year ) , I. Th ( -0.33 % / year ) , and I. Sp ( 0.59 % / year ) .
	manualset3
182550	2	414061	7	NULL	NULL	0	NULL	age	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	These trends with age were also expressed as annual rates of change : ABV/TV ( -0.52 % / year ) , I. Th ( -0.33 % / year ) , and I. Sp ( 0.59 % / year ) .
	manualset3
182551	3	414061	7	NULL	NULL	0	NULL	annual rates of change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These trends with age were also expressed as annual rates of change : ABV/TV ( -0.52 % / year ) , I. Th ( -0.33 % / year ) , and I. Sp ( 0.59 % / year ) .
	manualset3
182552	4	414061	7	NULL	NULL	0	NULL	ABV/TV ( -0.52 % / year )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These trends with age were also expressed as annual rates of change : ABV/TV ( -0.52 % / year ) , I. Th ( -0.33 % / year ) , and I. Sp ( 0.59 % / year ) .
	manualset3
182553	5	414061	7	NULL	NULL	0	NULL	 I. Th ( -0.33 % / year ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These trends with age were also expressed as annual rates of change : ABV/TV ( -0.52 % / year ) , I. Th ( -0.33 % / year ) , and I. Sp ( 0.59 % / year ) .
	manualset3
182554	6	414061	7	NULL	NULL	0	NULL	I. Sp ( 0.59 % / year ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These trends with age were also expressed as annual rates of change : ABV/TV ( -0.52 % / year ) , I. Th ( -0.33 % / year ) , and I. Sp ( 0.59 % / year ) .
	manualset3
182555	1	414062	7	NULL	NULL	0	NULL	two events	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These two events may account for the high activity of photosystem I and for the low content of chlorophyll b in the plastids .
	manualset3
182556	2	414062	7	NULL	NULL	0	NULL	high activity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These two events may account for the high activity of photosystem I and for the low content of chlorophyll b in the plastids .
	manualset3
182557	3	414062	7	NULL	NULL	NULL	NULL	photosystem I	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These two events may account for the high activity of photosystem I and for the low content of chlorophyll b in the plastids .
	manualset3
182558	4	414062	7	NULL	NULL	0	NULL	low content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These two events may account for the high activity of photosystem I and for the low content of chlorophyll b in the plastids .
	manualset3
182559	5	414062	7	NULL	NULL	0	NULL	chlorophyll b	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	These two events may account for the high activity of photosystem I and for the low content of chlorophyll b in the plastids .
	manualset3
182560	6	414062	7	NULL	NULL	0	NULL	plastids	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These two events may account for the high activity of photosystem I and for the low content of chlorophyll b in the plastids .
	manualset3
182561	1	414063	7	NULL	NULL	0	NULL	 two groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These two groups presented poorer quality chromatin , as evidenced fundamentally by a lower degree of condensation .
	manualset3
182562	2	414063	7	NULL	NULL	0	NULL	poorer quality chromatin	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These two groups presented poorer quality chromatin , as evidenced fundamentally by a lower degree of condensation .
	manualset3
182563	3	414063	7	NULL	NULL	0	NULL	lower degree	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These two groups presented poorer quality chromatin , as evidenced fundamentally by a lower degree of condensation .
	manualset3
182564	4	414063	7	NULL	NULL	0	NULL	condensation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These two groups presented poorer quality chromatin , as evidenced fundamentally by a lower degree of condensation .
	manualset3
182565	1	414064	7	NULL	NULL	NULL	NULL	two haplotypes 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These two haplotypes were strongly associated with the capacity of lines to respond to the environment ( genotype-environment interaction ) in ADH activity .
	manualset3
182566	2	414064	7	NULL	NULL	NULL	NULL	 capacity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These two haplotypes were strongly associated with the capacity of lines to respond to the environment ( genotype-environment interaction ) in ADH activity .
	manualset3
182567	3	414064	7	NULL	NULL	0	NULL	environment 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These two haplotypes were strongly associated with the capacity of lines to respond to the environment ( genotype-environment interaction ) in ADH activity .
	manualset3
182568	4	414064	7	NULL	NULL	0	NULL	genotype-environment interaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These two haplotypes were strongly associated with the capacity of lines to respond to the environment ( genotype-environment interaction ) in ADH activity .
	manualset3
182569	5	414064	7	NULL	NULL	0	NULL	ADH activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These two haplotypes were strongly associated with the capacity of lines to respond to the environment ( genotype-environment interaction ) in ADH activity .
	manualset3
184476	6	414064	7	NULL	NULL	0	NULL	lines	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These two haplotypes were strongly associated with the capacity of lines to respond to the environment ( genotype-environment interaction ) in ADH activity .
	manualset3
182570	1	414065	7	NULL	NULL	0	NULL	two intercalates	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These two intercalates also exhibit , rather surprisingly , perfect ordering in layer stacking without the displacement disorder , characteristic of many intercalated layered structures .
	manualset3
182571	2	414065	7	NULL	NULL	NULL	NULL	ordering in layer stacking	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These two intercalates also exhibit , rather surprisingly , perfect ordering in layer stacking without the displacement disorder , characteristic of many intercalated layered structures .
	manualset3
182572	3	414065	7	NULL	NULL	0	NULL	displacement disorder	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These two intercalates also exhibit , rather surprisingly , perfect ordering in layer stacking without the displacement disorder , characteristic of many intercalated layered structures .
	manualset3
182573	4	414065	7	NULL	NULL	0	NULL	intercalated layered structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These two intercalates also exhibit , rather surprisingly , perfect ordering in layer stacking without the displacement disorder , characteristic of many intercalated layered structures .
	manualset3
182581	1	414066	7	NULL	NULL	0	NULL	unique features	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These unique features allow the use of OCT to assess patients with acute coronary syndrome and to study the dynamic nature of coronary atherosclerosis in vivo and over time .
	manualset3
182582	2	414066	7	NULL	NULL	0	NULL	 use	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These unique features allow the use of OCT to assess patients with acute coronary syndrome and to study the dynamic nature of coronary atherosclerosis in vivo and over time .
	manualset3
182583	3	414066	7	NULL	NULL	0	NULL	OCT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These unique features allow the use of OCT to assess patients with acute coronary syndrome and to study the dynamic nature of coronary atherosclerosis in vivo and over time .
	manualset3
182584	4	414066	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These unique features allow the use of OCT to assess patients with acute coronary syndrome and to study the dynamic nature of coronary atherosclerosis in vivo and over time .
	manualset3
182585	5	414066	7	NULL	NULL	0	NULL	acute coronary syndrome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These unique features allow the use of OCT to assess patients with acute coronary syndrome and to study the dynamic nature of coronary atherosclerosis in vivo and over time .
	manualset3
182586	6	414066	7	NULL	NULL	0	NULL	dynamic nature	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These unique features allow the use of OCT to assess patients with acute coronary syndrome and to study the dynamic nature of coronary atherosclerosis in vivo and over time .
	manualset3
182587	7	414066	7	NULL	NULL	0	NULL	coronary atherosclerosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These unique features allow the use of OCT to assess patients with acute coronary syndrome and to study the dynamic nature of coronary atherosclerosis in vivo and over time .
	manualset3
182588	8	414066	7	NULL	NULL	0	NULL	 time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	These unique features allow the use of OCT to assess patients with acute coronary syndrome and to study the dynamic nature of coronary atherosclerosis in vivo and over time .
	manualset3
182589	1	414067	7	NULL	NULL	0	NULL	units 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	These units are connected via the carboxyl-ate O atoms and water mol-ecules , building polymeric layers parallel to ( 100 ) .
	manualset3
182590	2	414067	7	NULL	NULL	0	NULL	carboxyl-ate O atoms	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	These units are connected via the carboxyl-ate O atoms and water mol-ecules , building polymeric layers parallel to ( 100 ) .
	manualset3
182591	3	414067	7	NULL	NULL	0	NULL	water mol-ecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	These units are connected via the carboxyl-ate O atoms and water mol-ecules , building polymeric layers parallel to ( 100 ) .
	manualset3
182592	4	414067	7	NULL	NULL	0	NULL	polymeric layers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These units are connected via the carboxyl-ate O atoms and water mol-ecules , building polymeric layers parallel to ( 100 ) .
	manualset3
182593	5	414067	7	NULL	NULL	0	NULL	100	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These units are connected via the carboxyl-ate O atoms and water mol-ecules , building polymeric layers parallel to ( 100 ) .
	manualset3
182594	1	414068	7	NULL	NULL	0	NULL	values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These values increased during successive stages of development from dormant spore to vegetative bacillus , and they could be directly related to increases in cell water content .
	manualset3
182595	2	414068	7	NULL	NULL	0	NULL	successive stages	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	These values increased during successive stages of development from dormant spore to vegetative bacillus , and they could be directly related to increases in cell water content .
	manualset3
182596	3	414068	7	NULL	NULL	0	NULL	development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These values increased during successive stages of development from dormant spore to vegetative bacillus , and they could be directly related to increases in cell water content .
	manualset3
182597	4	414068	7	NULL	NULL	0	NULL	dormant spore	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These values increased during successive stages of development from dormant spore to vegetative bacillus , and they could be directly related to increases in cell water content .
	manualset3
182598	5	414068	7	NULL	NULL	0	NULL	vegetative bacillus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These values increased during successive stages of development from dormant spore to vegetative bacillus , and they could be directly related to increases in cell water content .
	manualset3
182599	6	414068	7	NULL	NULL	0	NULL	cell water content	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	These values increased during successive stages of development from dormant spore to vegetative bacillus , and they could be directly related to increases in cell water content .
	manualset3
182600	1	414069	7	NULL	NULL	0	NULL	well defined models	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These well defined models have left open the possibility that other betalactams can also induce specific reactions which implies that for diagnostic purposes , in addition to classical determinants , others are required for in vitro and/or in vivo evaluation .
	manualset3
182601	2	414069	7	NULL	NULL	0	NULL	possibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These well defined models have left open the possibility that other betalactams can also induce specific reactions which implies that for diagnostic purposes , in addition to classical determinants , others are required for in vitro and/or in vivo evaluation .
	manualset3
182602	3	414069	7	NULL	NULL	0	NULL	betalactams	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These well defined models have left open the possibility that other betalactams can also induce specific reactions which implies that for diagnostic purposes , in addition to classical determinants , others are required for in vitro and/or in vivo evaluation .
	manualset3
182603	4	414069	7	NULL	NULL	0	NULL	reactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These well defined models have left open the possibility that other betalactams can also induce specific reactions which implies that for diagnostic purposes , in addition to classical determinants , others are required for in vitro and/or in vivo evaluation .
	manualset3
182604	5	414069	7	NULL	NULL	0	NULL	diagnostic purposes	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These well defined models have left open the possibility that other betalactams can also induce specific reactions which implies that for diagnostic purposes , in addition to classical determinants , others are required for in vitro and/or in vivo evaluation .
	manualset3
182605	6	414069	7	NULL	NULL	0	NULL	addition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These well defined models have left open the possibility that other betalactams can also induce specific reactions which implies that for diagnostic purposes , in addition to classical determinants , others are required for in vitro and/or in vivo evaluation .
	manualset3
182606	7	414069	7	NULL	NULL	0	NULL	 classical determinants	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These well defined models have left open the possibility that other betalactams can also induce specific reactions which implies that for diagnostic purposes , in addition to classical determinants , others are required for in vitro and/or in vivo evaluation .
	manualset3
182607	8	414069	7	NULL	NULL	0	NULL	in vitro evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These well defined models have left open the possibility that other betalactams can also induce specific reactions which implies that for diagnostic purposes , in addition to classical determinants , others are required for in vitro and/or in vivo evaluation .
	manualset3
182608	9	414069	7	NULL	NULL	0	NULL	in vivo evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These well defined models have left open the possibility that other betalactams can also induce specific reactions which implies that for diagnostic purposes , in addition to classical determinants , others are required for in vitro and/or in vivo evaluation .
	manualset3
182609	1	414070	7	NULL	NULL	NULL	NULL	diamino , bisPEG	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These were diamino , bisPEG ( M ( w ) = 1300 ) ; triamino , trisPEG ( Mw = 1946 ) ; tetraamino , tetraPEG ( M ( w ) = 3956 ) ; monocarboxy , diamino , bisPEG ( M ( w ) = 1346 ) ; and monocarboxy , tetraamino , tetraPEG ( M ( w ) = 3999 ) .
	manualset3
182610	3	414070	7	NULL	NULL	NULL	NULL	triamino , trisPEG	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These were diamino , bisPEG ( M ( w ) = 1300 ) ; triamino , trisPEG ( Mw = 1946 ) ; tetraamino , tetraPEG ( M ( w ) = 3956 ) ; monocarboxy , diamino , bisPEG ( M ( w ) = 1346 ) ; and monocarboxy , tetraamino , tetraPEG ( M ( w ) = 3999 ) .
	manualset3
182611	2	414070	7	NULL	NULL	NULL	NULL	( M ( w ) = 1300 )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These were diamino , bisPEG ( M ( w ) = 1300 ) ; triamino , trisPEG ( Mw = 1946 ) ; tetraamino , tetraPEG ( M ( w ) = 3956 ) ; monocarboxy , diamino , bisPEG ( M ( w ) = 1346 ) ; and monocarboxy , tetraamino , tetraPEG ( M ( w ) = 3999 ) .
	manualset3
182612	4	414070	7	NULL	NULL	0	NULL	( Mw = 1946 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These were diamino , bisPEG ( M ( w ) = 1300 ) ; triamino , trisPEG ( Mw = 1946 ) ; tetraamino , tetraPEG ( M ( w ) = 3956 ) ; monocarboxy , diamino , bisPEG ( M ( w ) = 1346 ) ; and monocarboxy , tetraamino , tetraPEG ( M ( w ) = 3999 ) .
	manualset3
182613	5	414070	7	NULL	NULL	0	NULL	tetraamino , tetraPEG	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These were diamino , bisPEG ( M ( w ) = 1300 ) ; triamino , trisPEG ( Mw = 1946 ) ; tetraamino , tetraPEG ( M ( w ) = 3956 ) ; monocarboxy , diamino , bisPEG ( M ( w ) = 1346 ) ; and monocarboxy , tetraamino , tetraPEG ( M ( w ) = 3999 ) .
	manualset3
182615	6	414070	7	NULL	NULL	0	NULL	( M ( w ) = 3956 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These were diamino , bisPEG ( M ( w ) = 1300 ) ; triamino , trisPEG ( Mw = 1946 ) ; tetraamino , tetraPEG ( M ( w ) = 3956 ) ; monocarboxy , diamino , bisPEG ( M ( w ) = 1346 ) ; and monocarboxy , tetraamino , tetraPEG ( M ( w ) = 3999 ) .
	manualset3
182617	7	414070	7	NULL	NULL	0	NULL	monocarboxy , diamino , bisPEG	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These were diamino , bisPEG ( M ( w ) = 1300 ) ; triamino , trisPEG ( Mw = 1946 ) ; tetraamino , tetraPEG ( M ( w ) = 3956 ) ; monocarboxy , diamino , bisPEG ( M ( w ) = 1346 ) ; and monocarboxy , tetraamino , tetraPEG ( M ( w ) = 3999 ) .
	manualset3
182618	8	414070	7	NULL	NULL	0	NULL	( M ( w ) = 1346 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These were diamino , bisPEG ( M ( w ) = 1300 ) ; triamino , trisPEG ( Mw = 1946 ) ; tetraamino , tetraPEG ( M ( w ) = 3956 ) ; monocarboxy , diamino , bisPEG ( M ( w ) = 1346 ) ; and monocarboxy , tetraamino , tetraPEG ( M ( w ) = 3999 ) .
	manualset3
182620	9	414070	7	NULL	NULL	0	NULL	monocarboxy , tetraamino , tetraPEG	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These were diamino , bisPEG ( M ( w ) = 1300 ) ; triamino , trisPEG ( Mw = 1946 ) ; tetraamino , tetraPEG ( M ( w ) = 3956 ) ; monocarboxy , diamino , bisPEG ( M ( w ) = 1346 ) ; and monocarboxy , tetraamino , tetraPEG ( M ( w ) = 3999 ) .
	manualset3
182621	10	414070	7	NULL	NULL	0	NULL	( M ( w ) = 3999 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These were diamino , bisPEG ( M ( w ) = 1300 ) ; triamino , trisPEG ( Mw = 1946 ) ; tetraamino , tetraPEG ( M ( w ) = 3956 ) ; monocarboxy , diamino , bisPEG ( M ( w ) = 1346 ) ; and monocarboxy , tetraamino , tetraPEG ( M ( w ) = 3999 ) .
	manualset3
182622	1	414071	7	NULL	NULL	0	NULL	methylprednisolone pulse therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These were dramatically improved by methylprednisolone pulse therapy ( 30 mg/kg per day , for 3 days ) and CMV high titer immunoglobulin ( 400 mg/kg per day , for 3 days ) .
	manualset3
182623	2	414071	7	NULL	NULL	NULL	NULL	30 mg/kg per day 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These were dramatically improved by methylprednisolone pulse therapy ( 30 mg/kg per day , for 3 days ) and CMV high titer immunoglobulin ( 400 mg/kg per day , for 3 days ) .
	manualset3
182624	3	414071	7	NULL	NULL	NULL	NULL	CMV high titer immunoglobulin	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These were dramatically improved by methylprednisolone pulse therapy ( 30 mg/kg per day , for 3 days ) and CMV high titer immunoglobulin ( 400 mg/kg per day , for 3 days ) .
	manualset3
182625	4	414071	7	NULL	NULL	NULL	NULL	400 mg/kg per day 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These were dramatically improved by methylprednisolone pulse therapy ( 30 mg/kg per day , for 3 days ) and CMV high titer immunoglobulin ( 400 mg/kg per day , for 3 days ) .
	manualset3
182628	5	414071	7	NULL	NULL	0	NULL	3 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	These were dramatically improved by methylprednisolone pulse therapy ( 30 mg/kg per day , for 3 days ) and CMV high titer immunoglobulin ( 400 mg/kg per day , for 3 days ) .
	manualset3
182633	6	414071	7	NULL	NULL	0	NULL	3 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	These were dramatically improved by methylprednisolone pulse therapy ( 30 mg/kg per day , for 3 days ) and CMV high titer immunoglobulin ( 400 mg/kg per day , for 3 days ) .
	manualset3
182635	1	414072	7	NULL	NULL	0	NULL	mediator-specific changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , mediator-specific changes in the kinetics and magnitude of C/EBP mRNA expression pattern and profile of DNA-protein interactions were observed .
	manualset3
182637	2	414072	7	NULL	NULL	0	NULL	kinetics	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , mediator-specific changes in the kinetics and magnitude of C/EBP mRNA expression pattern and profile of DNA-protein interactions were observed .
	manualset3
182640	3	414072	7	NULL	NULL	0	NULL	magnitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , mediator-specific changes in the kinetics and magnitude of C/EBP mRNA expression pattern and profile of DNA-protein interactions were observed .
	manualset3
182641	4	414072	7	NULL	NULL	0	NULL	C/EBP mRNA expression pattern	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , mediator-specific changes in the kinetics and magnitude of C/EBP mRNA expression pattern and profile of DNA-protein interactions were observed .
	manualset3
182644	5	414072	7	NULL	NULL	0	NULL	profile	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , mediator-specific changes in the kinetics and magnitude of C/EBP mRNA expression pattern and profile of DNA-protein interactions were observed .
	manualset3
182646	6	414072	7	NULL	NULL	0	NULL	DNA-protein interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , mediator-specific changes in the kinetics and magnitude of C/EBP mRNA expression pattern and profile of DNA-protein interactions were observed .
	manualset3
182650	1	414073	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These women may need contraception as well as relief from perimenopausal symptoms .
	manualset3
182652	2	414073	7	NULL	NULL	0	NULL	contraception	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These women may need contraception as well as relief from perimenopausal symptoms .
	manualset3
182654	3	414073	7	NULL	NULL	0	NULL	perimenopausal symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These women may need contraception as well as relief from perimenopausal symptoms .
	manualset3
184458	4	414073	7	NULL	NULL	0	NULL	relief	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These women may need contraception as well as relief from perimenopausal symptoms .
	manualset3
182657	1	414074	7	NULL	NULL	0	NULL	works 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These works give IL-6 / sIL-6R alpha complex an important role in the biology of IL-6 .
	manualset3
182658	2	414074	7	NULL	NULL	0	NULL	IL-6 / sIL-6R alpha complex 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These works give IL-6 / sIL-6R alpha complex an important role in the biology of IL-6 .
	manualset3
182659	3	414074	7	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These works give IL-6 / sIL-6R alpha complex an important role in the biology of IL-6 .
	manualset3
182660	4	414074	7	NULL	NULL	0	NULL	 biology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These works give IL-6 / sIL-6R alpha complex an important role in the biology of IL-6 .
	manualset3
182661	5	414074	7	NULL	NULL	0	NULL	IL-6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These works give IL-6 / sIL-6R alpha complex an important role in the biology of IL-6 .
	manualset3
182662	1	414075	7	NULL	NULL	0	NULL	 baseline levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	They all returned to baseline levels by 60 days .
	manualset3
182663	2	414075	7	NULL	NULL	0	NULL	 60 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	They all returned to baseline levels by 60 days .
	manualset3
182756	1	414076	7	NULL	NULL	0	NULL	immune system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	They allow the immune system to make qualitatively distinct responses against different microbial infections .
	manualset3
182758	2	414076	7	NULL	NULL	0	NULL	 responses 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They allow the immune system to make qualitatively distinct responses against different microbial infections .
	manualset3
182760	3	414076	7	NULL	NULL	0	NULL	microbial infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	They allow the immune system to make qualitatively distinct responses against different microbial infections .
	manualset3
182762	1	414077	7	NULL	NULL	0	NULL	primary culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	They also indicate that primary culture of hepatocytes is a good model for further studies on insulin-like growth factor II gene regulation .
	manualset3
182763	2	414077	7	NULL	NULL	0	NULL	hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	They also indicate that primary culture of hepatocytes is a good model for further studies on insulin-like growth factor II gene regulation .
	manualset3
182764	3	414077	7	NULL	NULL	0	NULL	good model	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	They also indicate that primary culture of hepatocytes is a good model for further studies on insulin-like growth factor II gene regulation .
	manualset3
182766	4	414077	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	They also indicate that primary culture of hepatocytes is a good model for further studies on insulin-like growth factor II gene regulation .
	manualset3
182768	5	414077	7	NULL	NULL	0	NULL	insulin-like growth factor II gene regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They also indicate that primary culture of hepatocytes is a good model for further studies on insulin-like growth factor II gene regulation .
	manualset3
182772	1	414078	7	NULL	NULL	0	NULL	beta1 - / beta2-adrenergic increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	They also negatively modulate the beta1 - / beta2-adrenergic increase in inotropy and chronotropy , and reinforce the ( pre - and post-synaptic ) vagal control of cardiac contraction , thereby protecting the heart against excessive stimulation by catecholamines .
	manualset3
182779	2	414078	7	NULL	NULL	NULL	NULL	 inotropy 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	They also negatively modulate the beta1 - / beta2-adrenergic increase in inotropy and chronotropy , and reinforce the ( pre - and post-synaptic ) vagal control of cardiac contraction , thereby protecting the heart against excessive stimulation by catecholamines .
	manualset3
182781	3	414078	7	NULL	NULL	0	NULL	chronotropy	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	They also negatively modulate the beta1 - / beta2-adrenergic increase in inotropy and chronotropy , and reinforce the ( pre - and post-synaptic ) vagal control of cardiac contraction , thereby protecting the heart against excessive stimulation by catecholamines .
	manualset3
182784	4	414078	7	NULL	NULL	0	NULL	pre-synaptic vagal control	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They also negatively modulate the beta1 - / beta2-adrenergic increase in inotropy and chronotropy , and reinforce the ( pre - and post-synaptic ) vagal control of cardiac contraction , thereby protecting the heart against excessive stimulation by catecholamines .
	manualset3
182786	5	414078	7	NULL	NULL	0	NULL	post-synaptic vagal control	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They also negatively modulate the beta1 - / beta2-adrenergic increase in inotropy and chronotropy , and reinforce the ( pre - and post-synaptic ) vagal control of cardiac contraction , thereby protecting the heart against excessive stimulation by catecholamines .
	manualset3
182788	6	414078	7	NULL	NULL	0	NULL	cardiac contraction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They also negatively modulate the beta1 - / beta2-adrenergic increase in inotropy and chronotropy , and reinforce the ( pre - and post-synaptic ) vagal control of cardiac contraction , thereby protecting the heart against excessive stimulation by catecholamines .
	manualset3
182789	7	414078	7	NULL	NULL	0	NULL	 heart	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	They also negatively modulate the beta1 - / beta2-adrenergic increase in inotropy and chronotropy , and reinforce the ( pre - and post-synaptic ) vagal control of cardiac contraction , thereby protecting the heart against excessive stimulation by catecholamines .
	manualset3
182791	8	414078	7	NULL	NULL	0	NULL	excessive stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They also negatively modulate the beta1 - / beta2-adrenergic increase in inotropy and chronotropy , and reinforce the ( pre - and post-synaptic ) vagal control of cardiac contraction , thereby protecting the heart against excessive stimulation by catecholamines .
	manualset3
182792	9	414078	7	NULL	NULL	0	NULL	catecholamines 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	They also negatively modulate the beta1 - / beta2-adrenergic increase in inotropy and chronotropy , and reinforce the ( pre - and post-synaptic ) vagal control of cardiac contraction , thereby protecting the heart against excessive stimulation by catecholamines .
	manualset3
182796	1	414079	7	NULL	NULL	0	NULL	 naloxone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , naloxone ( 0.5 and 1.0 mM ) did not influence the binding of FITC-triflavin to platelet glycoprotein ( GP ) IIb/IIIa complex .
	manualset3
182798	2	414079	7	NULL	NULL	NULL	NULL	0.5 mM	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Additionally , naloxone ( 0.5 and 1.0 mM ) did not influence the binding of FITC-triflavin to platelet glycoprotein ( GP ) IIb/IIIa complex .
	manualset3
182799	3	414079	7	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , naloxone ( 0.5 and 1.0 mM ) did not influence the binding of FITC-triflavin to platelet glycoprotein ( GP ) IIb/IIIa complex .
	manualset3
182800	4	414079	7	NULL	NULL	0	NULL	FITC-triflavin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , naloxone ( 0.5 and 1.0 mM ) did not influence the binding of FITC-triflavin to platelet glycoprotein ( GP ) IIb/IIIa complex .
	manualset3
182802	5	414079	7	NULL	NULL	0	NULL	platelet glycoprotein ( GP ) IIb/IIIa complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , naloxone ( 0.5 and 1.0 mM ) did not influence the binding of FITC-triflavin to platelet glycoprotein ( GP ) IIb/IIIa complex .
	manualset3
184459	6	414079	7	NULL	NULL	0	NULL	1.0 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , naloxone ( 0.5 and 1.0 mM ) did not influence the binding of FITC-triflavin to platelet glycoprotein ( GP ) IIb/IIIa complex .
	manualset3
182826	1	414080	7	NULL	NULL	0	NULL	role 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They also play an important role in the development of the thymus and in the survival of thymocytes .
	manualset3
182827	2	414080	7	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They also play an important role in the development of the thymus and in the survival of thymocytes .
	manualset3
182828	3	414080	7	NULL	NULL	0	NULL	thymus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	They also play an important role in the development of the thymus and in the survival of thymocytes .
	manualset3
182829	4	414080	7	NULL	NULL	0	NULL	survival 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They also play an important role in the development of the thymus and in the survival of thymocytes .
	manualset3
182830	5	414080	7	NULL	NULL	0	NULL	thymocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	They also play an important role in the development of the thymus and in the survival of thymocytes .
	manualset3
182831	1	414081	7	NULL	NULL	0	NULL	 organizational procedures	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	They also should know how to initiate the organizational procedures to provide explantation , rapid procuration , and transportation of the explanted organs based upon to the regulations of TPG .
	manualset3
182832	2	414081	7	NULL	NULL	0	NULL	explantation	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	They also should know how to initiate the organizational procedures to provide explantation , rapid procuration , and transportation of the explanted organs based upon to the regulations of TPG .
	manualset3
182833	3	414081	7	NULL	NULL	0	NULL	rapid procuration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They also should know how to initiate the organizational procedures to provide explantation , rapid procuration , and transportation of the explanted organs based upon to the regulations of TPG .
	manualset3
182834	4	414081	7	NULL	NULL	0	NULL	transportation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They also should know how to initiate the organizational procedures to provide explantation , rapid procuration , and transportation of the explanted organs based upon to the regulations of TPG .
	manualset3
182836	5	414081	7	NULL	NULL	0	NULL	explanted organs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	They also should know how to initiate the organizational procedures to provide explantation , rapid procuration , and transportation of the explanted organs based upon to the regulations of TPG .
	manualset3
182839	6	414081	7	NULL	NULL	0	NULL	regulations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They also should know how to initiate the organizational procedures to provide explantation , rapid procuration , and transportation of the explanted organs based upon to the regulations of TPG .
	manualset3
182840	7	414081	7	NULL	NULL	0	NULL	TPG	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	They also should know how to initiate the organizational procedures to provide explantation , rapid procuration , and transportation of the explanted organs based upon to the regulations of TPG .
	manualset3
182846	1	414082	7	NULL	NULL	0	NULL	sexual education	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They also suggest that sexual and contraceptive education and counseling need to be cognizant of these differences since pre-coital experience may function as both a mechanism to prolong abstinence and to promote a gradual acceptance of one 's sexuality .
	manualset3
182847	2	414082	7	NULL	NULL	0	NULL	contraceptive education	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They also suggest that sexual and contraceptive education and counseling need to be cognizant of these differences since pre-coital experience may function as both a mechanism to prolong abstinence and to promote a gradual acceptance of one 's sexuality .
	manualset3
182848	3	414082	7	NULL	NULL	0	NULL	counseling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They also suggest that sexual and contraceptive education and counseling need to be cognizant of these differences since pre-coital experience may function as both a mechanism to prolong abstinence and to promote a gradual acceptance of one 's sexuality .
	manualset3
182849	4	414082	7	NULL	NULL	0	NULL	pre-coital experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They also suggest that sexual and contraceptive education and counseling need to be cognizant of these differences since pre-coital experience may function as both a mechanism to prolong abstinence and to promote a gradual acceptance of one 's sexuality .
	manualset3
182850	5	414082	7	NULL	NULL	0	NULL	function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They also suggest that sexual and contraceptive education and counseling need to be cognizant of these differences since pre-coital experience may function as both a mechanism to prolong abstinence and to promote a gradual acceptance of one 's sexuality .
	manualset3
182851	6	414082	7	NULL	NULL	0	NULL	mechanism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They also suggest that sexual and contraceptive education and counseling need to be cognizant of these differences since pre-coital experience may function as both a mechanism to prolong abstinence and to promote a gradual acceptance of one 's sexuality .
	manualset3
182852	7	414082	7	NULL	NULL	0	NULL	abstinence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	They also suggest that sexual and contraceptive education and counseling need to be cognizant of these differences since pre-coital experience may function as both a mechanism to prolong abstinence and to promote a gradual acceptance of one 's sexuality .
	manualset3
182853	8	414082	7	NULL	NULL	0	NULL	gradual acceptance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They also suggest that sexual and contraceptive education and counseling need to be cognizant of these differences since pre-coital experience may function as both a mechanism to prolong abstinence and to promote a gradual acceptance of one 's sexuality .
	manualset3
182854	9	414082	7	NULL	NULL	0	NULL	one 's sexuality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	They also suggest that sexual and contraceptive education and counseling need to be cognizant of these differences since pre-coital experience may function as both a mechanism to prolong abstinence and to promote a gradual acceptance of one 's sexuality .
	manualset3
184460	10	414082	7	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	They also suggest that sexual and contraceptive education and counseling need to be cognizant of these differences since pre-coital experience may function as both a mechanism to prolong abstinence and to promote a gradual acceptance of one 's sexuality .
	manualset3
182861	1	414083	7	NULL	NULL	0	NULL	intrinsically disordered `` hub proteins ''	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	They appear to act as intrinsically disordered `` hub proteins '' that integrate the activities of a range of transcription factors with a number of histone modifying enzymes .
	manualset3
182862	2	414083	7	NULL	NULL	0	NULL	activities 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They appear to act as intrinsically disordered `` hub proteins '' that integrate the activities of a range of transcription factors with a number of histone modifying enzymes .
	manualset3
182863	3	414083	7	NULL	NULL	0	NULL	range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	They appear to act as intrinsically disordered `` hub proteins '' that integrate the activities of a range of transcription factors with a number of histone modifying enzymes .
	manualset3
182864	4	414083	7	NULL	NULL	0	NULL	 transcription factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	They appear to act as intrinsically disordered `` hub proteins '' that integrate the activities of a range of transcription factors with a number of histone modifying enzymes .
	manualset3
182865	5	414083	7	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	They appear to act as intrinsically disordered `` hub proteins '' that integrate the activities of a range of transcription factors with a number of histone modifying enzymes .
	manualset3
182866	6	414083	7	NULL	NULL	0	NULL	histone modifying enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	They appear to act as intrinsically disordered `` hub proteins '' that integrate the activities of a range of transcription factors with a number of histone modifying enzymes .
	manualset3
182867	1	414084	7	NULL	NULL	0	NULL	 concept of `` curvature ''	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	They apply directly only after the concept of `` curvature '' is normalized and propagation is made to look perpendicular to activation fronts by rescaling distances to achieve isotropy .
	manualset3
182868	2	414084	7	NULL	NULL	0	NULL	propagation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They apply directly only after the concept of `` curvature '' is normalized and propagation is made to look perpendicular to activation fronts by rescaling distances to achieve isotropy .
	manualset3
182869	3	414084	7	NULL	NULL	0	NULL	activation fronts	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	They apply directly only after the concept of `` curvature '' is normalized and propagation is made to look perpendicular to activation fronts by rescaling distances to achieve isotropy .
	manualset3
182870	4	414084	7	NULL	NULL	0	NULL	rescaling distances 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	They apply directly only after the concept of `` curvature '' is normalized and propagation is made to look perpendicular to activation fronts by rescaling distances to achieve isotropy .
	manualset3
182871	5	414084	7	NULL	NULL	0	NULL	isotropy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They apply directly only after the concept of `` curvature '' is normalized and propagation is made to look perpendicular to activation fronts by rescaling distances to achieve isotropy .
	manualset3
182872	6	414084	7	NULL	NULL	0	NULL	perpendicular	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	They apply directly only after the concept of `` curvature '' is normalized and propagation is made to look perpendicular to activation fronts by rescaling distances to achieve isotropy .
	manualset3
182873	1	414085	7	NULL	NULL	0	NULL	antidiabetic bioactivities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They are also linked with antidiabetic bioactivities and have been associated with the reduction of obesity .
	manualset3
182874	2	414085	7	NULL	NULL	NULL	NULL	reduction	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	They are also linked with antidiabetic bioactivities and have been associated with the reduction of obesity .
	manualset3
182875	3	414085	7	NULL	NULL	0	NULL	obesity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	They are also linked with antidiabetic bioactivities and have been associated with the reduction of obesity .
	manualset3
182876	1	414086	7	NULL	NULL	0	NULL	Comparative study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative study of the biological properties of influenza virus strains , types A , Al , and B isolated in Tashkent ) .
	manualset3
182877	2	414086	7	NULL	NULL	0	NULL	biological properties	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative study of the biological properties of influenza virus strains , types A , Al , and B isolated in Tashkent ) .
	manualset3
182878	3	414086	7	NULL	NULL	0	NULL	influenza virus strains , types A	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative study of the biological properties of influenza virus strains , types A , Al , and B isolated in Tashkent ) .
	manualset3
182879	4	414086	7	NULL	NULL	0	NULL	influenza virus strains , types Al	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative study of the biological properties of influenza virus strains , types A , Al , and B isolated in Tashkent ) .
	manualset3
182880	5	414086	7	NULL	NULL	0	NULL	influenza virus strains , types B	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative study of the biological properties of influenza virus strains , types A , Al , and B isolated in Tashkent ) .
	manualset3
182881	6	414086	7	NULL	NULL	0	NULL	Tashkent 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative study of the biological properties of influenza virus strains , types A , Al , and B isolated in Tashkent ) .
	manualset3
182882	1	414087	7	NULL	NULL	0	NULL	niacin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , niacin selectively increases the plasma levels of Lp-AI ( HDL subfraction without apo AII ) , a cardioprotective subfraction of HDL in patients with low HDL .
	manualset3
182883	2	414087	7	NULL	NULL	0	NULL	 plasma levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , niacin selectively increases the plasma levels of Lp-AI ( HDL subfraction without apo AII ) , a cardioprotective subfraction of HDL in patients with low HDL .
	manualset3
182884	3	414087	7	NULL	NULL	0	NULL	Lp-AI ( HDL subfraction without apo AII )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , niacin selectively increases the plasma levels of Lp-AI ( HDL subfraction without apo AII ) , a cardioprotective subfraction of HDL in patients with low HDL .
	manualset3
182885	4	414087	7	NULL	NULL	0	NULL	cardioprotective subfraction	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , niacin selectively increases the plasma levels of Lp-AI ( HDL subfraction without apo AII ) , a cardioprotective subfraction of HDL in patients with low HDL .
	manualset3
182886	5	414087	7	NULL	NULL	0	NULL	HDL	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , niacin selectively increases the plasma levels of Lp-AI ( HDL subfraction without apo AII ) , a cardioprotective subfraction of HDL in patients with low HDL .
	manualset3
182887	6	414087	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , niacin selectively increases the plasma levels of Lp-AI ( HDL subfraction without apo AII ) , a cardioprotective subfraction of HDL in patients with low HDL .
	manualset3
182888	7	414087	7	NULL	NULL	0	NULL	low HDL	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , niacin selectively increases the plasma levels of Lp-AI ( HDL subfraction without apo AII ) , a cardioprotective subfraction of HDL in patients with low HDL .
	manualset3
182889	1	414088	7	NULL	NULL	0	NULL	collections	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They are collections of ribonucleoprotein complexes that , in most cases , remain still uncharacterized , except the processing bodies ( PBs ) and stress granules ( SGs ) , which have been studied ( and reviewed ) in detail .
	manualset3
182890	2	414088	7	NULL	NULL	0	NULL	 ribonucleoprotein complexes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	They are collections of ribonucleoprotein complexes that , in most cases , remain still uncharacterized , except the processing bodies ( PBs ) and stress granules ( SGs ) , which have been studied ( and reviewed ) in detail .
	manualset3
182891	3	414088	7	NULL	NULL	0	NULL	cases	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	They are collections of ribonucleoprotein complexes that , in most cases , remain still uncharacterized , except the processing bodies ( PBs ) and stress granules ( SGs ) , which have been studied ( and reviewed ) in detail .
	manualset3
182892	4	414088	7	NULL	NULL	0	NULL	processing bodies ( PBs )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	They are collections of ribonucleoprotein complexes that , in most cases , remain still uncharacterized , except the processing bodies ( PBs ) and stress granules ( SGs ) , which have been studied ( and reviewed ) in detail .
	manualset3
182893	5	414088	7	NULL	NULL	0	NULL	stress granules ( SGs )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	They are collections of ribonucleoprotein complexes that , in most cases , remain still uncharacterized , except the processing bodies ( PBs ) and stress granules ( SGs ) , which have been studied ( and reviewed ) in detail .
	manualset3
182901	1	414089	7	NULL	NULL	0	NULL	 12 identical subunits	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	They are composed of 12 identical subunits assembled with 23-symmetry to form a compact cage-like structure known to be stable at temperatures ) 70 degrees C and over a wide pH range .
	manualset3
182902	2	414089	7	NULL	NULL	0	NULL	23-symmetry	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	They are composed of 12 identical subunits assembled with 23-symmetry to form a compact cage-like structure known to be stable at temperatures ) 70 degrees C and over a wide pH range .
	manualset3
182903	3	414089	7	NULL	NULL	0	NULL	compact cage-like structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	They are composed of 12 identical subunits assembled with 23-symmetry to form a compact cage-like structure known to be stable at temperatures ) 70 degrees C and over a wide pH range .
	manualset3
182905	4	414089	7	NULL	NULL	0	NULL	temperatures ) 70 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	They are composed of 12 identical subunits assembled with 23-symmetry to form a compact cage-like structure known to be stable at temperatures ) 70 degrees C and over a wide pH range .
	manualset3
182907	5	414089	7	NULL	NULL	0	NULL	 pH range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	They are composed of 12 identical subunits assembled with 23-symmetry to form a compact cage-like structure known to be stable at temperatures ) 70 degrees C and over a wide pH range .
	manualset3
182909	1	414090	7	NULL	NULL	0	NULL	 members	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	They are distinguished from other members of the team only by role , not by expectation .
	manualset3
182910	2	414090	7	NULL	NULL	0	NULL	 team	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	They are distinguished from other members of the team only by role , not by expectation .
	manualset3
182911	3	414090	7	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They are distinguished from other members of the team only by role , not by expectation .
	manualset3
182913	4	414090	7	NULL	NULL	0	NULL	expectation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They are distinguished from other members of the team only by role , not by expectation .
	manualset3
182919	1	414091	7	NULL	NULL	0	NULL	side of the toxin molecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	They are located on the same side of the toxin molecule and the distance between their alpha-carbons is 2.7 nm .
	manualset3
182920	2	414091	7	NULL	NULL	0	NULL	distance	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	They are located on the same side of the toxin molecule and the distance between their alpha-carbons is 2.7 nm .
	manualset3
182922	3	414091	7	NULL	NULL	0	NULL	alpha-carbons	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	They are located on the same side of the toxin molecule and the distance between their alpha-carbons is 2.7 nm .
	manualset3
182925	4	414091	7	NULL	NULL	0	NULL	2.7 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	They are located on the same side of the toxin molecule and the distance between their alpha-carbons is 2.7 nm .
	manualset3
182928	1	414092	7	NULL	NULL	0	NULL	asymptomatics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	They are most often asymptomatics but carry a risk of long-term complications which can justify , in some cases , a treatment .
	manualset3
182929	2	414092	7	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	They are most often asymptomatics but carry a risk of long-term complications which can justify , in some cases , a treatment .
	manualset3
182930	3	414092	7	NULL	NULL	0	NULL	long-term complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	They are most often asymptomatics but carry a risk of long-term complications which can justify , in some cases , a treatment .
	manualset3
182931	4	414092	7	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	They are most often asymptomatics but carry a risk of long-term complications which can justify , in some cases , a treatment .
	manualset3
182932	5	414092	7	NULL	NULL	0	NULL	 treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	They are most often asymptomatics but carry a risk of long-term complications which can justify , in some cases , a treatment .
	manualset3
182933	1	414093	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , one of the HPV-16 gene products , the E6 oncogene , regulates TR2 gene expression .
	manualset3
182934	2	414093	7	NULL	NULL	0	NULL	HPV-16 gene products	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , one of the HPV-16 gene products , the E6 oncogene , regulates TR2 gene expression .
	manualset3
182935	3	414093	7	NULL	NULL	0	NULL	E6 oncogene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , one of the HPV-16 gene products , the E6 oncogene , regulates TR2 gene expression .
	manualset3
182936	4	414093	7	NULL	NULL	0	NULL	TR2 gene expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , one of the HPV-16 gene products , the E6 oncogene , regulates TR2 gene expression .
	manualset3
182941	1	414094	7	NULL	NULL	0	NULL	original excellent results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	They are somewhat disappointing and do not confirm the original excellent results reported in Germany for treatment of gallbladder stones .
	manualset3
182944	2	414094	7	NULL	NULL	0	NULL	Germany	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	They are somewhat disappointing and do not confirm the original excellent results reported in Germany for treatment of gallbladder stones .
	manualset3
182945	3	414094	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	They are somewhat disappointing and do not confirm the original excellent results reported in Germany for treatment of gallbladder stones .
	manualset3
182948	4	414094	7	NULL	NULL	0	NULL	gallbladder stones	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	They are somewhat disappointing and do not confirm the original excellent results reported in Germany for treatment of gallbladder stones .
	manualset3
182949	1	414095	7	NULL	NULL	0	NULL	monotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	They are used in monotherapy and as an adjunct to levodopa in early and advanced PD .
	manualset3
182950	2	414095	7	NULL	NULL	0	NULL	levodopa	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	They are used in monotherapy and as an adjunct to levodopa in early and advanced PD .
	manualset3
182951	3	414095	7	NULL	NULL	0	NULL	early PD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	They are used in monotherapy and as an adjunct to levodopa in early and advanced PD .
	manualset3
182952	4	414095	7	NULL	NULL	0	NULL	advanced PD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	They are used in monotherapy and as an adjunct to levodopa in early and advanced PD .
	manualset3
182954	1	414096	7	NULL	NULL	0	NULL	effect 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They assessed the effect of anti-angiogenic gene therapy for HCC treated by microbubble-enhanced US exposure and concluded that gene therapy mediated by US exposure enhanced by a microbubble contrast agent may become a new treatment option for HCC .
	manualset3
182955	2	414096	7	NULL	NULL	0	NULL	anti-angiogenic gene therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	They assessed the effect of anti-angiogenic gene therapy for HCC treated by microbubble-enhanced US exposure and concluded that gene therapy mediated by US exposure enhanced by a microbubble contrast agent may become a new treatment option for HCC .
	manualset3
182958	3	414096	7	NULL	NULL	0	NULL	HCC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	They assessed the effect of anti-angiogenic gene therapy for HCC treated by microbubble-enhanced US exposure and concluded that gene therapy mediated by US exposure enhanced by a microbubble contrast agent may become a new treatment option for HCC .
	manualset3
182960	4	414096	7	NULL	NULL	0	NULL	 microbubble-enhanced US exposure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	They assessed the effect of anti-angiogenic gene therapy for HCC treated by microbubble-enhanced US exposure and concluded that gene therapy mediated by US exposure enhanced by a microbubble contrast agent may become a new treatment option for HCC .
	manualset3
182961	5	414096	7	NULL	NULL	0	NULL	gene therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	They assessed the effect of anti-angiogenic gene therapy for HCC treated by microbubble-enhanced US exposure and concluded that gene therapy mediated by US exposure enhanced by a microbubble contrast agent may become a new treatment option for HCC .
	manualset3
182962	6	414096	7	NULL	NULL	0	NULL	US exposure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	They assessed the effect of anti-angiogenic gene therapy for HCC treated by microbubble-enhanced US exposure and concluded that gene therapy mediated by US exposure enhanced by a microbubble contrast agent may become a new treatment option for HCC .
	manualset3
182963	7	414096	7	NULL	NULL	0	NULL	microbubble contrast agent 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	They assessed the effect of anti-angiogenic gene therapy for HCC treated by microbubble-enhanced US exposure and concluded that gene therapy mediated by US exposure enhanced by a microbubble contrast agent may become a new treatment option for HCC .
	manualset3
182964	8	414096	7	NULL	NULL	0	NULL	new treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	They assessed the effect of anti-angiogenic gene therapy for HCC treated by microbubble-enhanced US exposure and concluded that gene therapy mediated by US exposure enhanced by a microbubble contrast agent may become a new treatment option for HCC .
	manualset3
182965	9	414096	7	NULL	NULL	0	NULL	HCC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	They assessed the effect of anti-angiogenic gene therapy for HCC treated by microbubble-enhanced US exposure and concluded that gene therapy mediated by US exposure enhanced by a microbubble contrast agent may become a new treatment option for HCC .
	manualset3
182975	1	414097	7	NULL	NULL	0	NULL	direct acylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They can be formed by direct acylation by asparaginyl-tRNA synthetase ( AsnRS ) or glutaminyl-tRNA synthetase ( GlnRS ) .
	manualset3
182976	2	414097	7	NULL	NULL	0	NULL	asparaginyl-tRNA synthetase ( AsnRS )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	They can be formed by direct acylation by asparaginyl-tRNA synthetase ( AsnRS ) or glutaminyl-tRNA synthetase ( GlnRS ) .
	manualset3
182977	3	414097	7	NULL	NULL	0	NULL	glutaminyl-tRNA synthetase ( GlnRS )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	They can be formed by direct acylation by asparaginyl-tRNA synthetase ( AsnRS ) or glutaminyl-tRNA synthetase ( GlnRS ) .
	manualset3
182978	1	414098	7	NULL	NULL	0	NULL	effector T cell responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They can control both effector and regulatory T cell responses and their activity can in turn be modulated by these interactions .
	manualset3
182979	2	414098	7	NULL	NULL	0	NULL	 regulatory T cell responses 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They can control both effector and regulatory T cell responses and their activity can in turn be modulated by these interactions .
	manualset3
182980	3	414098	7	NULL	NULL	0	NULL	activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They can control both effector and regulatory T cell responses and their activity can in turn be modulated by these interactions .
	manualset3
182981	4	414098	7	NULL	NULL	0	NULL	 interactions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They can control both effector and regulatory T cell responses and their activity can in turn be modulated by these interactions .
	manualset3
182982	1	414099	7	NULL	NULL	0	NULL	signals	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They can transmit signals from cell to cell , locally or at a distance through the circulation .
	manualset3
182983	2	414099	7	NULL	NULL	0	NULL	 cell 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	They can transmit signals from cell to cell , locally or at a distance through the circulation .
	manualset3
182984	3	414099	7	NULL	NULL	0	NULL	cell 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	They can transmit signals from cell to cell , locally or at a distance through the circulation .
	manualset3
182985	4	414099	7	NULL	NULL	0	NULL	distance	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	They can transmit signals from cell to cell , locally or at a distance through the circulation .
	manualset3
182986	5	414099	7	NULL	NULL	0	NULL	circulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They can transmit signals from cell to cell , locally or at a distance through the circulation .
	manualset3
182987	1	414100	7	NULL	NULL	0	NULL	words	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	They can understand words and running speech better when using the cochlear implant with lip-reading compared to lip-reading alone .
	manualset3
182988	2	414100	7	NULL	NULL	0	NULL	running speech 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They can understand words and running speech better when using the cochlear implant with lip-reading compared to lip-reading alone .
	manualset3
182989	3	414100	7	NULL	NULL	0	NULL	cochlear implant	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	They can understand words and running speech better when using the cochlear implant with lip-reading compared to lip-reading alone .
	manualset3
182990	4	414100	7	NULL	NULL	0	NULL	lip-reading	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They can understand words and running speech better when using the cochlear implant with lip-reading compared to lip-reading alone .
	manualset3
182991	5	414100	7	NULL	NULL	0	NULL	lip-reading	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They can understand words and running speech better when using the cochlear implant with lip-reading compared to lip-reading alone .
	manualset3
182992	1	414101	7	NULL	NULL	0	NULL	overexpression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , overexpression of dominant-negative ( dn ) Akt in C33A cells could inhibit the IL-6-induced increase of Mcl-1 .
	manualset3
182993	2	414101	7	NULL	NULL	0	NULL	dominant-negative ( dn ) Akt 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , overexpression of dominant-negative ( dn ) Akt in C33A cells could inhibit the IL-6-induced increase of Mcl-1 .
	manualset3
182994	3	414101	7	NULL	NULL	0	NULL	C33A cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , overexpression of dominant-negative ( dn ) Akt in C33A cells could inhibit the IL-6-induced increase of Mcl-1 .
	manualset3
182995	4	414101	7	NULL	NULL	0	NULL	IL-6-induced increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , overexpression of dominant-negative ( dn ) Akt in C33A cells could inhibit the IL-6-induced increase of Mcl-1 .
	manualset3
182996	5	414101	7	NULL	NULL	0	NULL	Mcl-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , overexpression of dominant-negative ( dn ) Akt in C33A cells could inhibit the IL-6-induced increase of Mcl-1 .
	manualset3
182997	1	414102	7	NULL	NULL	0	NULL	principles	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	They confirm the key principles of biosimilarity , namely stand alone manufacturing process development and demonstrated comparability , which are described in many existing regional guidelines for biosimilars .
	manualset3
182998	2	414102	7	NULL	NULL	0	NULL	biosimilarity	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	They confirm the key principles of biosimilarity , namely stand alone manufacturing process development and demonstrated comparability , which are described in many existing regional guidelines for biosimilars .
	manualset3
182999	3	414102	7	NULL	NULL	0	NULL	stand alone manufacturing process development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They confirm the key principles of biosimilarity , namely stand alone manufacturing process development and demonstrated comparability , which are described in many existing regional guidelines for biosimilars .
	manualset3
183000	4	414102	7	NULL	NULL	0	NULL	comparability	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	They confirm the key principles of biosimilarity , namely stand alone manufacturing process development and demonstrated comparability , which are described in many existing regional guidelines for biosimilars .
	manualset3
183001	5	414102	7	NULL	NULL	0	NULL	regional guidelines	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	They confirm the key principles of biosimilarity , namely stand alone manufacturing process development and demonstrated comparability , which are described in many existing regional guidelines for biosimilars .
	manualset3
183002	6	414102	7	NULL	NULL	0	NULL	biosimilars	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	They confirm the key principles of biosimilarity , namely stand alone manufacturing process development and demonstrated comparability , which are described in many existing regional guidelines for biosimilars .
	manualset3
183003	1	414103	7	NULL	NULL	0	NULL	stakeholders	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	They discuss how to support stakeholders in understanding and contributing to the development of an assessment system and how to meet some of the challenges they encountered .
	manualset3
183004	2	414103	7	NULL	NULL	0	NULL	understanding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They discuss how to support stakeholders in understanding and contributing to the development of an assessment system and how to meet some of the challenges they encountered .
	manualset3
183005	3	414103	7	NULL	NULL	0	NULL	contributing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They discuss how to support stakeholders in understanding and contributing to the development of an assessment system and how to meet some of the challenges they encountered .
	manualset3
183006	4	414103	7	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They discuss how to support stakeholders in understanding and contributing to the development of an assessment system and how to meet some of the challenges they encountered .
	manualset3
183007	5	414103	7	NULL	NULL	0	NULL	assessment system 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	They discuss how to support stakeholders in understanding and contributing to the development of an assessment system and how to meet some of the challenges they encountered .
	manualset3
183008	6	414103	7	NULL	NULL	0	NULL	challenges	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They discuss how to support stakeholders in understanding and contributing to the development of an assessment system and how to meet some of the challenges they encountered .
	manualset3
183009	1	414104	7	NULL	NULL	0	NULL	gifts	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	They enable us to recognize our own gifts , the needs of our people , the amazing and gracious traditions in which we stand , and the blessing that is always there in the midst of crisis .
	manualset3
183010	2	414104	7	NULL	NULL	0	NULL	needs of our people	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	They enable us to recognize our own gifts , the needs of our people , the amazing and gracious traditions in which we stand , and the blessing that is always there in the midst of crisis .
	manualset3
183011	3	414104	7	NULL	NULL	0	NULL	amazing and gracious traditions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They enable us to recognize our own gifts , the needs of our people , the amazing and gracious traditions in which we stand , and the blessing that is always there in the midst of crisis .
	manualset3
183012	4	414104	7	NULL	NULL	NULL	NULL	blessing	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	They enable us to recognize our own gifts , the needs of our people , the amazing and gracious traditions in which we stand , and the blessing that is always there in the midst of crisis .
	manualset3
183013	5	414104	7	NULL	NULL	NULL	NULL	midst of crisis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	They enable us to recognize our own gifts , the needs of our people , the amazing and gracious traditions in which we stand , and the blessing that is always there in the midst of crisis .
	manualset3
183014	1	414105	7	NULL	NULL	0	NULL	phyletic lines	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	They formed distinct phyletic lines in the Actinomadura 16S rRNA gene tree and were closely associated with the type strains of Actinomadura meyerae ( sequence similarity of 98.3-98 .5 % ) , Actinomadura napierensis ( 98.1-98 .3 % ) and Actinomadura latina ( 96.4-96 .8 % ) .
	manualset3
183015	2	414105	7	NULL	NULL	0	NULL	Actinomadura 16S rRNA gene tree	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	They formed distinct phyletic lines in the Actinomadura 16S rRNA gene tree and were closely associated with the type strains of Actinomadura meyerae ( sequence similarity of 98.3-98 .5 % ) , Actinomadura napierensis ( 98.1-98 .3 % ) and Actinomadura latina ( 96.4-96 .8 % ) .
	manualset3
183016	3	414105	7	NULL	NULL	0	NULL	strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	They formed distinct phyletic lines in the Actinomadura 16S rRNA gene tree and were closely associated with the type strains of Actinomadura meyerae ( sequence similarity of 98.3-98 .5 % ) , Actinomadura napierensis ( 98.1-98 .3 % ) and Actinomadura latina ( 96.4-96 .8 % ) .
	manualset3
183017	4	414105	7	NULL	NULL	0	NULL	Actinomadura meyerae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	They formed distinct phyletic lines in the Actinomadura 16S rRNA gene tree and were closely associated with the type strains of Actinomadura meyerae ( sequence similarity of 98.3-98 .5 % ) , Actinomadura napierensis ( 98.1-98 .3 % ) and Actinomadura latina ( 96.4-96 .8 % ) .
	manualset3
183018	5	414105	7	NULL	NULL	NULL	NULL	sequence similarity 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	They formed distinct phyletic lines in the Actinomadura 16S rRNA gene tree and were closely associated with the type strains of Actinomadura meyerae ( sequence similarity of 98.3-98 .5 % ) , Actinomadura napierensis ( 98.1-98 .3 % ) and Actinomadura latina ( 96.4-96 .8 % ) .
	manualset3
183019	6	414105	7	NULL	NULL	0	NULL	 Actinomadura napierensis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	They formed distinct phyletic lines in the Actinomadura 16S rRNA gene tree and were closely associated with the type strains of Actinomadura meyerae ( sequence similarity of 98.3-98 .5 % ) , Actinomadura napierensis ( 98.1-98 .3 % ) and Actinomadura latina ( 96.4-96 .8 % ) .
	manualset3
183020	7	414105	7	NULL	NULL	0	NULL	98.1-98 .3 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	They formed distinct phyletic lines in the Actinomadura 16S rRNA gene tree and were closely associated with the type strains of Actinomadura meyerae ( sequence similarity of 98.3-98 .5 % ) , Actinomadura napierensis ( 98.1-98 .3 % ) and Actinomadura latina ( 96.4-96 .8 % ) .
	manualset3
183021	8	414105	7	NULL	NULL	0	NULL	Actinomadura latina	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	They formed distinct phyletic lines in the Actinomadura 16S rRNA gene tree and were closely associated with the type strains of Actinomadura meyerae ( sequence similarity of 98.3-98 .5 % ) , Actinomadura napierensis ( 98.1-98 .3 % ) and Actinomadura latina ( 96.4-96 .8 % ) .
	manualset3
183022	9	414105	7	NULL	NULL	0	NULL	96.4-96 .8 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	They formed distinct phyletic lines in the Actinomadura 16S rRNA gene tree and were closely associated with the type strains of Actinomadura meyerae ( sequence similarity of 98.3-98 .5 % ) , Actinomadura napierensis ( 98.1-98 .3 % ) and Actinomadura latina ( 96.4-96 .8 % ) .
	manualset3
183364	10	414105	7	NULL	NULL	0	NULL	98.3-98 .5 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	They formed distinct phyletic lines in the Actinomadura 16S rRNA gene tree and were closely associated with the type strains of Actinomadura meyerae ( sequence similarity of 98.3-98 .5 % ) , Actinomadura napierensis ( 98.1-98 .3 % ) and Actinomadura latina ( 96.4-96 .8 % ) .
	manualset3
183023	1	414106	7	NULL	NULL	0	NULL	phenotype	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	They have a similar phenotype including moderate skeletal fragility with several femur fractures , dentinogenesis imperfecta , wormian bone , and reduced height and weight .
	manualset3
183024	2	414106	7	NULL	NULL	0	NULL	moderate skeletal fragility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	They have a similar phenotype including moderate skeletal fragility with several femur fractures , dentinogenesis imperfecta , wormian bone , and reduced height and weight .
	manualset3
183025	3	414106	7	NULL	NULL	0	NULL	several femur fractures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	They have a similar phenotype including moderate skeletal fragility with several femur fractures , dentinogenesis imperfecta , wormian bone , and reduced height and weight .
	manualset3
183026	4	414106	7	NULL	NULL	0	NULL	dentinogenesis imperfecta	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	They have a similar phenotype including moderate skeletal fragility with several femur fractures , dentinogenesis imperfecta , wormian bone , and reduced height and weight .
	manualset3
183027	5	414106	7	NULL	NULL	0	NULL	wormian bone	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	They have a similar phenotype including moderate skeletal fragility with several femur fractures , dentinogenesis imperfecta , wormian bone , and reduced height and weight .
	manualset3
183028	6	414106	7	NULL	NULL	0	NULL	reduced height	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	They have a similar phenotype including moderate skeletal fragility with several femur fractures , dentinogenesis imperfecta , wormian bone , and reduced height and weight .
	manualset3
183029	7	414106	7	NULL	NULL	0	NULL	 reduced weight	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	They have a similar phenotype including moderate skeletal fragility with several femur fractures , dentinogenesis imperfecta , wormian bone , and reduced height and weight .
	manualset3
183030	1	414107	7	NULL	NULL	0	NULL	suppression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , suppression mediated by Treg appears to be mediated , in part , by the induction of apoptosis in the CD4 + CD25 - effector cell .
	manualset3
183031	2	414107	7	NULL	NULL	0	NULL	Treg	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , suppression mediated by Treg appears to be mediated , in part , by the induction of apoptosis in the CD4 + CD25 - effector cell .
	manualset3
183032	3	414107	7	NULL	NULL	0	NULL	induction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , suppression mediated by Treg appears to be mediated , in part , by the induction of apoptosis in the CD4 + CD25 - effector cell .
	manualset3
183033	4	414107	7	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , suppression mediated by Treg appears to be mediated , in part , by the induction of apoptosis in the CD4 + CD25 - effector cell .
	manualset3
183034	5	414107	7	NULL	NULL	0	NULL	CD4 + CD25 - effector cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , suppression mediated by Treg appears to be mediated , in part , by the induction of apoptosis in the CD4 + CD25 - effector cell .
	manualset3
183365	1	414108	7	NULL	NULL	0	NULL	`` weigh ''	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	They have considered and assigned a `` weigh '' in % in one scale of priority ( number that follows the variable ) and beyond fifty descriptors of the productive system , constituting the total system .
	manualset3
183366	2	414108	7	NULL	NULL	0	NULL	%	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	They have considered and assigned a `` weigh '' in % in one scale of priority ( number that follows the variable ) and beyond fifty descriptors of the productive system , constituting the total system .
	manualset3
183367	3	414108	7	NULL	NULL	0	NULL	one scale of priority	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	They have considered and assigned a `` weigh '' in % in one scale of priority ( number that follows the variable ) and beyond fifty descriptors of the productive system , constituting the total system .
	manualset3
183368	4	414108	7	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	They have considered and assigned a `` weigh '' in % in one scale of priority ( number that follows the variable ) and beyond fifty descriptors of the productive system , constituting the total system .
	manualset3
183369	5	414108	7	NULL	NULL	0	NULL	variable	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	They have considered and assigned a `` weigh '' in % in one scale of priority ( number that follows the variable ) and beyond fifty descriptors of the productive system , constituting the total system .
	manualset3
183370	6	414108	7	NULL	NULL	0	NULL	fifty descriptors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	They have considered and assigned a `` weigh '' in % in one scale of priority ( number that follows the variable ) and beyond fifty descriptors of the productive system , constituting the total system .
	manualset3
183371	7	414108	7	NULL	NULL	0	NULL	productive system	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	They have considered and assigned a `` weigh '' in % in one scale of priority ( number that follows the variable ) and beyond fifty descriptors of the productive system , constituting the total system .
	manualset3
183372	8	414108	7	NULL	NULL	0	NULL	total system 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	They have considered and assigned a `` weigh '' in % in one scale of priority ( number that follows the variable ) and beyond fifty descriptors of the productive system , constituting the total system .
	manualset3
183373	1	414109	7	NULL	NULL	0	NULL	arthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	They have developed arthritis , which in one brother has required chronic treatment ; and persistent intermittent diarrhea , necessitating treatment for inflammatory bowel disease .
	manualset3
183374	2	414109	7	NULL	NULL	0	NULL	brother	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	They have developed arthritis , which in one brother has required chronic treatment ; and persistent intermittent diarrhea , necessitating treatment for inflammatory bowel disease .
	manualset3
183375	3	414109	7	NULL	NULL	0	NULL	chronic treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	They have developed arthritis , which in one brother has required chronic treatment ; and persistent intermittent diarrhea , necessitating treatment for inflammatory bowel disease .
	manualset3
183376	4	414109	7	NULL	NULL	0	NULL	persistent intermittent diarrhea	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	They have developed arthritis , which in one brother has required chronic treatment ; and persistent intermittent diarrhea , necessitating treatment for inflammatory bowel disease .
	manualset3
183377	5	414109	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	They have developed arthritis , which in one brother has required chronic treatment ; and persistent intermittent diarrhea , necessitating treatment for inflammatory bowel disease .
	manualset3
183378	6	414109	7	NULL	NULL	0	NULL	inflammatory bowel disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	They have developed arthritis , which in one brother has required chronic treatment ; and persistent intermittent diarrhea , necessitating treatment for inflammatory bowel disease .
	manualset3
183379	1	414110	7	NULL	NULL	0	NULL	high affinity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They have high affinity for IGF-I and - II .
	manualset3
183380	2	414110	7	NULL	NULL	0	NULL	IGF-I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	They have high affinity for IGF-I and - II .
	manualset3
183381	3	414110	7	NULL	NULL	0	NULL	IGF-II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	They have high affinity for IGF-I and - II .
	manualset3
183382	1	414111	7	NULL	NULL	0	NULL	issue	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183383	2	414111	7	NULL	NULL	0	NULL	 recommendations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183384	3	414111	7	NULL	NULL	0	NULL	reorganization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183385	4	414111	7	NULL	NULL	0	NULL	Russia 's laboratory tuberculosis diagnosis service	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183386	5	414111	7	NULL	NULL	0	NULL	laboratories	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183387	6	414111	7	NULL	NULL	0	NULL	up-to-date equipment	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183388	7	414111	7	NULL	NULL	0	NULL	full-scale training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183389	8	414111	7	NULL	NULL	0	NULL	laboratory workers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183390	9	414111	7	NULL	NULL	0	NULL	procedures	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183391	10	414111	7	NULL	NULL	0	NULL	microbiological tests 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183392	11	414111	7	NULL	NULL	0	NULL	tuberculosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183393	12	414111	7	NULL	NULL	0	NULL	 bacteriological tuberculosis service	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183394	13	414111	7	NULL	NULL	0	NULL	Russia	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183395	14	414111	7	NULL	NULL	0	NULL	monitoring	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183396	15	414111	7	NULL	NULL	0	NULL	tuberculosis-controlling facilities	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183397	16	414111	7	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183398	17	414111	7	NULL	NULL	0	NULL	normative documents	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183399	18	414111	7	NULL	NULL	0	NULL	current standards	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183400	19	414111	7	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183401	20	414111	7	NULL	NULL	0	NULL	working operations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183402	21	414111	7	NULL	NULL	0	NULL	criteria	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183403	22	414111	7	NULL	NULL	0	NULL	estimating 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183404	23	414111	7	NULL	NULL	0	NULL	load 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183405	24	414111	7	NULL	NULL	0	NULL	personnel	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183406	25	414111	7	NULL	NULL	0	NULL	procedures	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183407	26	414111	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183408	27	414111	7	NULL	NULL	0	NULL	new staff lists	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183409	28	414111	7	NULL	NULL	0	NULL	laboratories	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183410	29	414111	7	NULL	NULL	0	NULL	level 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183411	30	414111	7	NULL	NULL	0	NULL	structure of salaries	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183412	31	414111	7	NULL	NULL	0	NULL	laboratory 's personnel 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183413	32	414111	7	NULL	NULL	0	NULL	conclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They have made their conclusion on this issue and developed the following recommendations : to continue the reorganization of Russia 's laboratory tuberculosis diagnosis service ; to reconstruct and repair laboratories ; to provide them with up-to-date equipment ; to make a full-scale training of laboratory workers ; to standardize the procedures of microbiological tests for tuberculosis ; to organize bacteriological tuberculosis service monitoring in Russia , including monitoring of tuberculosis-controlling facilities ; to develop and officially approve a number of normative documents ( current standards for the time spent on working operations and criteria for estimating the load on the personnel performing the procedures of a study , new staff lists for laboratories , the level and structure of salaries in the laboratory 's personnel ) .
	manualset3
183414	1	414112	7	NULL	NULL	0	NULL	African American children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	They highlight the importance of targeting African American children and adolescents for prevention despite the fact that African American youth have the lowest rates of smoking across all ethnic groups .
	manualset3
183415	2	414112	7	NULL	NULL	0	NULL	adolescents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	They highlight the importance of targeting African American children and adolescents for prevention despite the fact that African American youth have the lowest rates of smoking across all ethnic groups .
	manualset3
183416	3	414112	7	NULL	NULL	0	NULL	prevention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They highlight the importance of targeting African American children and adolescents for prevention despite the fact that African American youth have the lowest rates of smoking across all ethnic groups .
	manualset3
183417	4	414112	7	NULL	NULL	0	NULL	African American youth	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	They highlight the importance of targeting African American children and adolescents for prevention despite the fact that African American youth have the lowest rates of smoking across all ethnic groups .
	manualset3
183418	5	414112	7	NULL	NULL	0	NULL	lowest rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	They highlight the importance of targeting African American children and adolescents for prevention despite the fact that African American youth have the lowest rates of smoking across all ethnic groups .
	manualset3
183419	6	414112	7	NULL	NULL	0	NULL	smoking 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	They highlight the importance of targeting African American children and adolescents for prevention despite the fact that African American youth have the lowest rates of smoking across all ethnic groups .
	manualset3
183420	7	414112	7	NULL	NULL	0	NULL	ethnic groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	They highlight the importance of targeting African American children and adolescents for prevention despite the fact that African American youth have the lowest rates of smoking across all ethnic groups .
	manualset3
183421	8	414112	7	NULL	NULL	0	NULL	 targeting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They highlight the importance of targeting African American children and adolescents for prevention despite the fact that African American youth have the lowest rates of smoking across all ethnic groups .
	manualset3
183422	1	414113	7	NULL	NULL	0	NULL	detection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	They include detection of outbreaks of hospital-acquired infections , screening for multi-resistant organisms , advice to clinicians about disinfection , sterilization and isolation procedures , and the rational use of antibiotics .
	manualset3
183423	2	414113	7	NULL	NULL	0	NULL	outbreaks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	They include detection of outbreaks of hospital-acquired infections , screening for multi-resistant organisms , advice to clinicians about disinfection , sterilization and isolation procedures , and the rational use of antibiotics .
	manualset3
183424	3	414113	7	NULL	NULL	0	NULL	hospital-acquired infections	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	They include detection of outbreaks of hospital-acquired infections , screening for multi-resistant organisms , advice to clinicians about disinfection , sterilization and isolation procedures , and the rational use of antibiotics .
	manualset3
183425	4	414113	7	NULL	NULL	0	NULL	screening	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	They include detection of outbreaks of hospital-acquired infections , screening for multi-resistant organisms , advice to clinicians about disinfection , sterilization and isolation procedures , and the rational use of antibiotics .
	manualset3
183426	5	414113	7	NULL	NULL	0	NULL	multi-resistant organisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	They include detection of outbreaks of hospital-acquired infections , screening for multi-resistant organisms , advice to clinicians about disinfection , sterilization and isolation procedures , and the rational use of antibiotics .
	manualset3
183427	6	414113	7	NULL	NULL	0	NULL	clinicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	They include detection of outbreaks of hospital-acquired infections , screening for multi-resistant organisms , advice to clinicians about disinfection , sterilization and isolation procedures , and the rational use of antibiotics .
	manualset3
183428	7	414113	7	NULL	NULL	0	NULL	disinfection 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	They include detection of outbreaks of hospital-acquired infections , screening for multi-resistant organisms , advice to clinicians about disinfection , sterilization and isolation procedures , and the rational use of antibiotics .
	manualset3
183429	8	414113	7	NULL	NULL	0	NULL	sterilization procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	They include detection of outbreaks of hospital-acquired infections , screening for multi-resistant organisms , advice to clinicians about disinfection , sterilization and isolation procedures , and the rational use of antibiotics .
	manualset3
183430	9	414113	7	NULL	NULL	0	NULL	isolation procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	They include detection of outbreaks of hospital-acquired infections , screening for multi-resistant organisms , advice to clinicians about disinfection , sterilization and isolation procedures , and the rational use of antibiotics .
	manualset3
183431	10	414113	7	NULL	NULL	0	NULL	rational use	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	They include detection of outbreaks of hospital-acquired infections , screening for multi-resistant organisms , advice to clinicians about disinfection , sterilization and isolation procedures , and the rational use of antibiotics .
	manualset3
183432	11	414113	7	NULL	NULL	0	NULL	 antibiotics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	They include detection of outbreaks of hospital-acquired infections , screening for multi-resistant organisms , advice to clinicians about disinfection , sterilization and isolation procedures , and the rational use of antibiotics .
	manualset3
183433	1	414114	7	NULL	NULL	NULL	NULL	ocular lesions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	They include ocular lesions leading to blindness .
	manualset3
183434	2	414114	7	NULL	NULL	0	NULL	blindness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	They include ocular lesions leading to blindness .
	manualset3
183435	1	414115	7	NULL	NULL	0	NULL	nature	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the nature of the insertion device , guaranteeing lack of contact between the transverse arm of the IUD and the vagina , assures the sterility of the IUD even at the moment of introduction into the uterus , limiting the transport of bacteria into the cavity .
	manualset3
183436	2	414115	7	NULL	NULL	0	NULL	insertion device	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the nature of the insertion device , guaranteeing lack of contact between the transverse arm of the IUD and the vagina , assures the sterility of the IUD even at the moment of introduction into the uterus , limiting the transport of bacteria into the cavity .
	manualset3
183437	3	414115	7	NULL	NULL	0	NULL	 lack of contact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the nature of the insertion device , guaranteeing lack of contact between the transverse arm of the IUD and the vagina , assures the sterility of the IUD even at the moment of introduction into the uterus , limiting the transport of bacteria into the cavity .
	manualset3
183438	4	414115	7	NULL	NULL	0	NULL	transverse arm	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the nature of the insertion device , guaranteeing lack of contact between the transverse arm of the IUD and the vagina , assures the sterility of the IUD even at the moment of introduction into the uterus , limiting the transport of bacteria into the cavity .
	manualset3
183439	5	414115	7	NULL	NULL	0	NULL	IUD	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the nature of the insertion device , guaranteeing lack of contact between the transverse arm of the IUD and the vagina , assures the sterility of the IUD even at the moment of introduction into the uterus , limiting the transport of bacteria into the cavity .
	manualset3
183440	6	414115	7	NULL	NULL	0	NULL	vagina	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the nature of the insertion device , guaranteeing lack of contact between the transverse arm of the IUD and the vagina , assures the sterility of the IUD even at the moment of introduction into the uterus , limiting the transport of bacteria into the cavity .
	manualset3
183441	7	414115	7	NULL	NULL	0	NULL	sterility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the nature of the insertion device , guaranteeing lack of contact between the transverse arm of the IUD and the vagina , assures the sterility of the IUD even at the moment of introduction into the uterus , limiting the transport of bacteria into the cavity .
	manualset3
183442	8	414115	7	NULL	NULL	0	NULL	IUD	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the nature of the insertion device , guaranteeing lack of contact between the transverse arm of the IUD and the vagina , assures the sterility of the IUD even at the moment of introduction into the uterus , limiting the transport of bacteria into the cavity .
	manualset3
183443	9	414115	7	NULL	NULL	0	NULL	introduction	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the nature of the insertion device , guaranteeing lack of contact between the transverse arm of the IUD and the vagina , assures the sterility of the IUD even at the moment of introduction into the uterus , limiting the transport of bacteria into the cavity .
	manualset3
183444	10	414115	7	NULL	NULL	0	NULL	uterus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the nature of the insertion device , guaranteeing lack of contact between the transverse arm of the IUD and the vagina , assures the sterility of the IUD even at the moment of introduction into the uterus , limiting the transport of bacteria into the cavity .
	manualset3
183445	11	414115	7	NULL	NULL	0	NULL	limiting	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the nature of the insertion device , guaranteeing lack of contact between the transverse arm of the IUD and the vagina , assures the sterility of the IUD even at the moment of introduction into the uterus , limiting the transport of bacteria into the cavity .
	manualset3
183446	12	414115	7	NULL	NULL	0	NULL	transport 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the nature of the insertion device , guaranteeing lack of contact between the transverse arm of the IUD and the vagina , assures the sterility of the IUD even at the moment of introduction into the uterus , limiting the transport of bacteria into the cavity .
	manualset3
183447	13	414115	7	NULL	NULL	0	NULL	bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the nature of the insertion device , guaranteeing lack of contact between the transverse arm of the IUD and the vagina , assures the sterility of the IUD even at the moment of introduction into the uterus , limiting the transport of bacteria into the cavity .
	manualset3
183448	14	414115	7	NULL	NULL	0	NULL	cavity	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the nature of the insertion device , guaranteeing lack of contact between the transverse arm of the IUD and the vagina , assures the sterility of the IUD even at the moment of introduction into the uterus , limiting the transport of bacteria into the cavity .
	manualset3
183449	1	414116	7	NULL	NULL	0	NULL	no amino acid sequence diversity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They indicate no amino acid sequence diversity according to peptide mapping , but differ in their redox state , as shown by free-sulfhydryl-group-specific cleavage at cysteine residues with 2-nitro-5-thiocyanobenzoic acid .
	manualset3
183450	2	414116	7	NULL	NULL	0	NULL	peptide mapping	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	They indicate no amino acid sequence diversity according to peptide mapping , but differ in their redox state , as shown by free-sulfhydryl-group-specific cleavage at cysteine residues with 2-nitro-5-thiocyanobenzoic acid .
	manualset3
183451	3	414116	7	NULL	NULL	0	NULL	redox state	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They indicate no amino acid sequence diversity according to peptide mapping , but differ in their redox state , as shown by free-sulfhydryl-group-specific cleavage at cysteine residues with 2-nitro-5-thiocyanobenzoic acid .
	manualset3
183452	4	414116	7	NULL	NULL	0	NULL	free-sulfhydryl-group-specific cleavage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They indicate no amino acid sequence diversity according to peptide mapping , but differ in their redox state , as shown by free-sulfhydryl-group-specific cleavage at cysteine residues with 2-nitro-5-thiocyanobenzoic acid .
	manualset3
183453	5	414116	7	NULL	NULL	0	NULL	cysteine residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	They indicate no amino acid sequence diversity according to peptide mapping , but differ in their redox state , as shown by free-sulfhydryl-group-specific cleavage at cysteine residues with 2-nitro-5-thiocyanobenzoic acid .
	manualset3
183454	6	414116	7	NULL	NULL	0	NULL	2-nitro-5-thiocyanobenzoic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	They indicate no amino acid sequence diversity according to peptide mapping , but differ in their redox state , as shown by free-sulfhydryl-group-specific cleavage at cysteine residues with 2-nitro-5-thiocyanobenzoic acid .
	manualset3
183455	1	414117	7	NULL	NULL	0	NULL	EMF exposure	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	They measured EMF exposure produced and , using validated computerized models , the authors exploited the data of one of the laptop computers ( LTCs ) to estimate the magnetic flux exposure of the user and of the fetus in the womb , when the laptop is used at close contact with the woman 's womb .
	manualset3
183456	2	414117	7	NULL	NULL	0	NULL	computerized models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	They measured EMF exposure produced and , using validated computerized models , the authors exploited the data of one of the laptop computers ( LTCs ) to estimate the magnetic flux exposure of the user and of the fetus in the womb , when the laptop is used at close contact with the woman 's womb .
	manualset3
183457	3	414117	7	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	They measured EMF exposure produced and , using validated computerized models , the authors exploited the data of one of the laptop computers ( LTCs ) to estimate the magnetic flux exposure of the user and of the fetus in the womb , when the laptop is used at close contact with the woman 's womb .
	manualset3
183458	4	414117	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	They measured EMF exposure produced and , using validated computerized models , the authors exploited the data of one of the laptop computers ( LTCs ) to estimate the magnetic flux exposure of the user and of the fetus in the womb , when the laptop is used at close contact with the woman 's womb .
	manualset3
183459	5	414117	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	They measured EMF exposure produced and , using validated computerized models , the authors exploited the data of one of the laptop computers ( LTCs ) to estimate the magnetic flux exposure of the user and of the fetus in the womb , when the laptop is used at close contact with the woman 's womb .
	manualset3
183460	6	414117	7	NULL	NULL	NULL	NULL	laptop computers ( LTCs )	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	They measured EMF exposure produced and , using validated computerized models , the authors exploited the data of one of the laptop computers ( LTCs ) to estimate the magnetic flux exposure of the user and of the fetus in the womb , when the laptop is used at close contact with the woman 's womb .
	manualset3
183461	7	414117	7	NULL	NULL	0	NULL	magnetic flux exposure	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	They measured EMF exposure produced and , using validated computerized models , the authors exploited the data of one of the laptop computers ( LTCs ) to estimate the magnetic flux exposure of the user and of the fetus in the womb , when the laptop is used at close contact with the woman 's womb .
	manualset3
183462	8	414117	7	NULL	NULL	0	NULL	user	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	They measured EMF exposure produced and , using validated computerized models , the authors exploited the data of one of the laptop computers ( LTCs ) to estimate the magnetic flux exposure of the user and of the fetus in the womb , when the laptop is used at close contact with the woman 's womb .
	manualset3
183463	9	414117	7	NULL	NULL	0	NULL	fetus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	They measured EMF exposure produced and , using validated computerized models , the authors exploited the data of one of the laptop computers ( LTCs ) to estimate the magnetic flux exposure of the user and of the fetus in the womb , when the laptop is used at close contact with the woman 's womb .
	manualset3
183464	10	414117	7	NULL	NULL	0	NULL	womb	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	They measured EMF exposure produced and , using validated computerized models , the authors exploited the data of one of the laptop computers ( LTCs ) to estimate the magnetic flux exposure of the user and of the fetus in the womb , when the laptop is used at close contact with the woman 's womb .
	manualset3
183465	11	414117	7	NULL	NULL	NULL	NULL	laptop	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	They measured EMF exposure produced and , using validated computerized models , the authors exploited the data of one of the laptop computers ( LTCs ) to estimate the magnetic flux exposure of the user and of the fetus in the womb , when the laptop is used at close contact with the woman 's womb .
	manualset3
183466	12	414117	7	NULL	NULL	0	NULL	close contact 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They measured EMF exposure produced and , using validated computerized models , the authors exploited the data of one of the laptop computers ( LTCs ) to estimate the magnetic flux exposure of the user and of the fetus in the womb , when the laptop is used at close contact with the woman 's womb .
	manualset3
183467	13	414117	7	NULL	NULL	0	NULL	woman 's womb	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	They measured EMF exposure produced and , using validated computerized models , the authors exploited the data of one of the laptop computers ( LTCs ) to estimate the magnetic flux exposure of the user and of the fetus in the womb , when the laptop is used at close contact with the woman 's womb .
	manualset3
183468	1	414118	7	NULL	NULL	0	NULL	CO2 reduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They photocatalyzed CO2 reduction to CO using a wide-range of visible light , and their photocatalytic abilities were strongly affected by the phosphorus ligands on the Re site .
	manualset3
183469	2	414118	7	NULL	NULL	NULL	NULL	CO	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	They photocatalyzed CO2 reduction to CO using a wide-range of visible light , and their photocatalytic abilities were strongly affected by the phosphorus ligands on the Re site .
	manualset3
183470	3	414118	7	NULL	NULL	0	NULL	 wide-range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	They photocatalyzed CO2 reduction to CO using a wide-range of visible light , and their photocatalytic abilities were strongly affected by the phosphorus ligands on the Re site .
	manualset3
183471	4	414118	7	NULL	NULL	0	NULL	visible light 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	They photocatalyzed CO2 reduction to CO using a wide-range of visible light , and their photocatalytic abilities were strongly affected by the phosphorus ligands on the Re site .
	manualset3
183472	5	414118	7	NULL	NULL	0	NULL	photocatalytic abilities 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They photocatalyzed CO2 reduction to CO using a wide-range of visible light , and their photocatalytic abilities were strongly affected by the phosphorus ligands on the Re site .
	manualset3
183473	6	414118	7	NULL	NULL	0	NULL	phosphorus ligands	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	They photocatalyzed CO2 reduction to CO using a wide-range of visible light , and their photocatalytic abilities were strongly affected by the phosphorus ligands on the Re site .
	manualset3
183474	7	414118	7	NULL	NULL	0	NULL	Re site	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	They photocatalyzed CO2 reduction to CO using a wide-range of visible light , and their photocatalytic abilities were strongly affected by the phosphorus ligands on the Re site .
	manualset3
183475	1	414119	7	NULL	NULL	0	NULL	wide array	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	They possess a wide array of spontaneous electrical activity ranging from slow oscillations of membrane potential to action potentials .
	manualset3
183476	2	414119	7	NULL	NULL	0	NULL	spontaneous electrical activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They possess a wide array of spontaneous electrical activity ranging from slow oscillations of membrane potential to action potentials .
	manualset3
183477	3	414119	7	NULL	NULL	0	NULL	slow oscillations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They possess a wide array of spontaneous electrical activity ranging from slow oscillations of membrane potential to action potentials .
	manualset3
183478	4	414119	7	NULL	NULL	0	NULL	membrane potential	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	They possess a wide array of spontaneous electrical activity ranging from slow oscillations of membrane potential to action potentials .
	manualset3
183479	5	414119	7	NULL	NULL	0	NULL	action potentials	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	They possess a wide array of spontaneous electrical activity ranging from slow oscillations of membrane potential to action potentials .
	manualset3
183480	1	414120	7	NULL	NULL	0	NULL	amplitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	They progressively declined in amplitude when elicited at frequencies of 0.05 Hz or more , and this is discussed in relation to studies on acetylcholine ( ACh ) output .6 .
	manualset3
183481	2	414120	7	NULL	NULL	0	NULL	 frequencies	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	They progressively declined in amplitude when elicited at frequencies of 0.05 Hz or more , and this is discussed in relation to studies on acetylcholine ( ACh ) output .6 .
	manualset3
183482	3	414120	7	NULL	NULL	0	NULL	 0.05 Hz 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	They progressively declined in amplitude when elicited at frequencies of 0.05 Hz or more , and this is discussed in relation to studies on acetylcholine ( ACh ) output .6 .
	manualset3
183483	4	414120	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	They progressively declined in amplitude when elicited at frequencies of 0.05 Hz or more , and this is discussed in relation to studies on acetylcholine ( ACh ) output .6 .
	manualset3
183484	5	414120	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	They progressively declined in amplitude when elicited at frequencies of 0.05 Hz or more , and this is discussed in relation to studies on acetylcholine ( ACh ) output .6 .
	manualset3
183485	6	414120	7	NULL	NULL	0	NULL	acetylcholine ( ACh ) output .6	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	They progressively declined in amplitude when elicited at frequencies of 0.05 Hz or more , and this is discussed in relation to studies on acetylcholine ( ACh ) output .6 .
	manualset3
183486	1	414121	7	NULL	NULL	0	NULL	regions	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	They remained stable solely in regions deprived of ECM , where they were submitted to lower tensional forces .
	manualset3
183487	2	414121	7	NULL	NULL	0	NULL	ECM	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	They remained stable solely in regions deprived of ECM , where they were submitted to lower tensional forces .
	manualset3
183488	3	414121	7	NULL	NULL	0	NULL	 lower tensional forces	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	They remained stable solely in regions deprived of ECM , where they were submitted to lower tensional forces .
	manualset3
183489	1	414122	7	NULL	NULL	0	NULL	disorder	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	They serve to detect a disorder of the end organ or of the hypothalamus-pituitary system ( determination of testosterone or estradiol , determination of LH and FSH before and after stimulation with the releasing hormone LHRH , determination of growth hormone before and after insulin and arginine , determination of TSH before and after TRH ) .
	manualset3
183490	2	414122	7	NULL	NULL	0	NULL	end organ	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	They serve to detect a disorder of the end organ or of the hypothalamus-pituitary system ( determination of testosterone or estradiol , determination of LH and FSH before and after stimulation with the releasing hormone LHRH , determination of growth hormone before and after insulin and arginine , determination of TSH before and after TRH ) .
	manualset3
183491	3	414122	7	NULL	NULL	0	NULL	hypothalamus-pituitary system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	They serve to detect a disorder of the end organ or of the hypothalamus-pituitary system ( determination of testosterone or estradiol , determination of LH and FSH before and after stimulation with the releasing hormone LHRH , determination of growth hormone before and after insulin and arginine , determination of TSH before and after TRH ) .
	manualset3
183492	4	414122	7	NULL	NULL	0	NULL	determination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	They serve to detect a disorder of the end organ or of the hypothalamus-pituitary system ( determination of testosterone or estradiol , determination of LH and FSH before and after stimulation with the releasing hormone LHRH , determination of growth hormone before and after insulin and arginine , determination of TSH before and after TRH ) .
	manualset3
183493	5	414122	7	NULL	NULL	0	NULL	testosterone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	They serve to detect a disorder of the end organ or of the hypothalamus-pituitary system ( determination of testosterone or estradiol , determination of LH and FSH before and after stimulation with the releasing hormone LHRH , determination of growth hormone before and after insulin and arginine , determination of TSH before and after TRH ) .
	manualset3
183494	6	414122	7	NULL	NULL	0	NULL	estradiol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	They serve to detect a disorder of the end organ or of the hypothalamus-pituitary system ( determination of testosterone or estradiol , determination of LH and FSH before and after stimulation with the releasing hormone LHRH , determination of growth hormone before and after insulin and arginine , determination of TSH before and after TRH ) .
	manualset3
183495	7	414122	7	NULL	NULL	0	NULL	determination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	They serve to detect a disorder of the end organ or of the hypothalamus-pituitary system ( determination of testosterone or estradiol , determination of LH and FSH before and after stimulation with the releasing hormone LHRH , determination of growth hormone before and after insulin and arginine , determination of TSH before and after TRH ) .
	manualset3
183496	8	414122	7	NULL	NULL	0	NULL	LH	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	They serve to detect a disorder of the end organ or of the hypothalamus-pituitary system ( determination of testosterone or estradiol , determination of LH and FSH before and after stimulation with the releasing hormone LHRH , determination of growth hormone before and after insulin and arginine , determination of TSH before and after TRH ) .
	manualset3
183497	9	414122	7	NULL	NULL	0	NULL	FSH	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	They serve to detect a disorder of the end organ or of the hypothalamus-pituitary system ( determination of testosterone or estradiol , determination of LH and FSH before and after stimulation with the releasing hormone LHRH , determination of growth hormone before and after insulin and arginine , determination of TSH before and after TRH ) .
	manualset3
183498	10	414122	7	NULL	NULL	0	NULL	before stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They serve to detect a disorder of the end organ or of the hypothalamus-pituitary system ( determination of testosterone or estradiol , determination of LH and FSH before and after stimulation with the releasing hormone LHRH , determination of growth hormone before and after insulin and arginine , determination of TSH before and after TRH ) .
	manualset3
183499	11	414122	7	NULL	NULL	0	NULL	after stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They serve to detect a disorder of the end organ or of the hypothalamus-pituitary system ( determination of testosterone or estradiol , determination of LH and FSH before and after stimulation with the releasing hormone LHRH , determination of growth hormone before and after insulin and arginine , determination of TSH before and after TRH ) .
	manualset3
183500	12	414122	7	NULL	NULL	0	NULL	releasing hormone LHRH	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	They serve to detect a disorder of the end organ or of the hypothalamus-pituitary system ( determination of testosterone or estradiol , determination of LH and FSH before and after stimulation with the releasing hormone LHRH , determination of growth hormone before and after insulin and arginine , determination of TSH before and after TRH ) .
	manualset3
183501	13	414122	7	NULL	NULL	0	NULL	determination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	They serve to detect a disorder of the end organ or of the hypothalamus-pituitary system ( determination of testosterone or estradiol , determination of LH and FSH before and after stimulation with the releasing hormone LHRH , determination of growth hormone before and after insulin and arginine , determination of TSH before and after TRH ) .
	manualset3
183502	14	414122	7	NULL	NULL	0	NULL	growth hormone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	They serve to detect a disorder of the end organ or of the hypothalamus-pituitary system ( determination of testosterone or estradiol , determination of LH and FSH before and after stimulation with the releasing hormone LHRH , determination of growth hormone before and after insulin and arginine , determination of TSH before and after TRH ) .
	manualset3
183503	15	414122	7	NULL	NULL	0	NULL	insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	They serve to detect a disorder of the end organ or of the hypothalamus-pituitary system ( determination of testosterone or estradiol , determination of LH and FSH before and after stimulation with the releasing hormone LHRH , determination of growth hormone before and after insulin and arginine , determination of TSH before and after TRH ) .
	manualset3
183504	16	414122	7	NULL	NULL	0	NULL	arginine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	They serve to detect a disorder of the end organ or of the hypothalamus-pituitary system ( determination of testosterone or estradiol , determination of LH and FSH before and after stimulation with the releasing hormone LHRH , determination of growth hormone before and after insulin and arginine , determination of TSH before and after TRH ) .
	manualset3
183505	17	414122	7	NULL	NULL	0	NULL	determination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	They serve to detect a disorder of the end organ or of the hypothalamus-pituitary system ( determination of testosterone or estradiol , determination of LH and FSH before and after stimulation with the releasing hormone LHRH , determination of growth hormone before and after insulin and arginine , determination of TSH before and after TRH ) .
	manualset3
183506	18	414122	7	NULL	NULL	0	NULL	TSH	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	They serve to detect a disorder of the end organ or of the hypothalamus-pituitary system ( determination of testosterone or estradiol , determination of LH and FSH before and after stimulation with the releasing hormone LHRH , determination of growth hormone before and after insulin and arginine , determination of TSH before and after TRH ) .
	manualset3
183507	19	414122	7	NULL	NULL	0	NULL	TRH 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	They serve to detect a disorder of the end organ or of the hypothalamus-pituitary system ( determination of testosterone or estradiol , determination of LH and FSH before and after stimulation with the releasing hormone LHRH , determination of growth hormone before and after insulin and arginine , determination of TSH before and after TRH ) .
	manualset3
183508	1	414123	7	NULL	NULL	0	NULL	seminars	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	They should be sent to seminars and training workshops .
	manualset3
183509	2	414123	7	NULL	NULL	0	NULL	training workshops 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	They should be sent to seminars and training workshops .
	manualset3
183510	1	414124	7	NULL	NULL	0	NULL	early diagnosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	They should be skilled in the early diagnosis of osteoarthritis and in the use of current common nonoperative treatments including patient education , activity modification , shoe modifications , braces , oral analgesics , oral nonsteroidal antiinflammatory medications , oral dietary supplements , and intraarticular injections .
	manualset3
183511	2	414124	7	NULL	NULL	0	NULL	osteoarthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	They should be skilled in the early diagnosis of osteoarthritis and in the use of current common nonoperative treatments including patient education , activity modification , shoe modifications , braces , oral analgesics , oral nonsteroidal antiinflammatory medications , oral dietary supplements , and intraarticular injections .
	manualset3
183512	3	414124	7	NULL	NULL	0	NULL	current common nonoperative treatments	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	They should be skilled in the early diagnosis of osteoarthritis and in the use of current common nonoperative treatments including patient education , activity modification , shoe modifications , braces , oral analgesics , oral nonsteroidal antiinflammatory medications , oral dietary supplements , and intraarticular injections .
	manualset3
183513	4	414124	7	NULL	NULL	0	NULL	patient education	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They should be skilled in the early diagnosis of osteoarthritis and in the use of current common nonoperative treatments including patient education , activity modification , shoe modifications , braces , oral analgesics , oral nonsteroidal antiinflammatory medications , oral dietary supplements , and intraarticular injections .
	manualset3
183514	5	414124	7	NULL	NULL	0	NULL	activity modification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They should be skilled in the early diagnosis of osteoarthritis and in the use of current common nonoperative treatments including patient education , activity modification , shoe modifications , braces , oral analgesics , oral nonsteroidal antiinflammatory medications , oral dietary supplements , and intraarticular injections .
	manualset3
183515	6	414124	7	NULL	NULL	0	NULL	shoe modifications 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They should be skilled in the early diagnosis of osteoarthritis and in the use of current common nonoperative treatments including patient education , activity modification , shoe modifications , braces , oral analgesics , oral nonsteroidal antiinflammatory medications , oral dietary supplements , and intraarticular injections .
	manualset3
183516	7	414124	7	NULL	NULL	0	NULL	braces	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	They should be skilled in the early diagnosis of osteoarthritis and in the use of current common nonoperative treatments including patient education , activity modification , shoe modifications , braces , oral analgesics , oral nonsteroidal antiinflammatory medications , oral dietary supplements , and intraarticular injections .
	manualset3
183517	8	414124	7	NULL	NULL	0	NULL	oral analgesics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	They should be skilled in the early diagnosis of osteoarthritis and in the use of current common nonoperative treatments including patient education , activity modification , shoe modifications , braces , oral analgesics , oral nonsteroidal antiinflammatory medications , oral dietary supplements , and intraarticular injections .
	manualset3
183518	9	414124	7	NULL	NULL	0	NULL	oral nonsteroidal antiinflammatory medications	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	They should be skilled in the early diagnosis of osteoarthritis and in the use of current common nonoperative treatments including patient education , activity modification , shoe modifications , braces , oral analgesics , oral nonsteroidal antiinflammatory medications , oral dietary supplements , and intraarticular injections .
	manualset3
183519	10	414124	7	NULL	NULL	0	NULL	oral dietary supplements 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	They should be skilled in the early diagnosis of osteoarthritis and in the use of current common nonoperative treatments including patient education , activity modification , shoe modifications , braces , oral analgesics , oral nonsteroidal antiinflammatory medications , oral dietary supplements , and intraarticular injections .
	manualset3
183520	11	414124	7	NULL	NULL	0	NULL	 intraarticular injections 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	They should be skilled in the early diagnosis of osteoarthritis and in the use of current common nonoperative treatments including patient education , activity modification , shoe modifications , braces , oral analgesics , oral nonsteroidal antiinflammatory medications , oral dietary supplements , and intraarticular injections .
	manualset3
183521	1	414125	7	NULL	NULL	0	NULL	selectivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They show that selectivity in favor of the actual substrate preQ ( 1 ) over preQ ( 0 ) is not achieved by a difference in affinity but via a higher turnover rate .
	manualset3
183522	2	414125	7	NULL	NULL	0	NULL	actual substrate preQ ( 1 )	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	They show that selectivity in favor of the actual substrate preQ ( 1 ) over preQ ( 0 ) is not achieved by a difference in affinity but via a higher turnover rate .
	manualset3
183523	3	414125	7	NULL	NULL	0	NULL	 preQ ( 0 ) 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	They show that selectivity in favor of the actual substrate preQ ( 1 ) over preQ ( 0 ) is not achieved by a difference in affinity but via a higher turnover rate .
	manualset3
183524	4	414125	7	NULL	NULL	0	NULL	affinity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They show that selectivity in favor of the actual substrate preQ ( 1 ) over preQ ( 0 ) is not achieved by a difference in affinity but via a higher turnover rate .
	manualset3
183525	5	414125	7	NULL	NULL	0	NULL	higher turnover rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	They show that selectivity in favor of the actual substrate preQ ( 1 ) over preQ ( 0 ) is not achieved by a difference in affinity but via a higher turnover rate .
	manualset3
184461	6	414125	7	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	They show that selectivity in favor of the actual substrate preQ ( 1 ) over preQ ( 0 ) is not achieved by a difference in affinity but via a higher turnover rate .
	manualset3
184477	7	414125	7	NULL	NULL	0	NULL	favor	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They show that selectivity in favor of the actual substrate preQ ( 1 ) over preQ ( 0 ) is not achieved by a difference in affinity but via a higher turnover rate .
	manualset3
183526	1	414126	7	NULL	NULL	0	NULL	GDP-bound inactive state 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	They shuttle between the GDP-bound inactive state and the GTP-bound activated state and their activation is predominantly mediated by a family of guanine nucleotide exchange factors ( GEFs ) referred to as ROPGEFs .
	manualset3
183527	2	414126	7	NULL	NULL	0	NULL	GTP-bound activated state	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	They shuttle between the GDP-bound inactive state and the GTP-bound activated state and their activation is predominantly mediated by a family of guanine nucleotide exchange factors ( GEFs ) referred to as ROPGEFs .
	manualset3
183528	3	414126	7	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They shuttle between the GDP-bound inactive state and the GTP-bound activated state and their activation is predominantly mediated by a family of guanine nucleotide exchange factors ( GEFs ) referred to as ROPGEFs .
	manualset3
183529	4	414126	7	NULL	NULL	0	NULL	 family 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	They shuttle between the GDP-bound inactive state and the GTP-bound activated state and their activation is predominantly mediated by a family of guanine nucleotide exchange factors ( GEFs ) referred to as ROPGEFs .
	manualset3
183530	5	414126	7	NULL	NULL	0	NULL	guanine nucleotide exchange factors ( GEFs )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	They shuttle between the GDP-bound inactive state and the GTP-bound activated state and their activation is predominantly mediated by a family of guanine nucleotide exchange factors ( GEFs ) referred to as ROPGEFs .
	manualset3
183531	6	414126	7	NULL	NULL	0	NULL	ROPGEFs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	They shuttle between the GDP-bound inactive state and the GTP-bound activated state and their activation is predominantly mediated by a family of guanine nucleotide exchange factors ( GEFs ) referred to as ROPGEFs .
	manualset3
183532	1	414127	7	NULL	NULL	0	NULL	peanut lectin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	They were all labeled by peanut lectin ( Arachis hypogaea ) and three showed reactivity for S-100 protein .
	manualset3
183533	2	414127	7	NULL	NULL	0	NULL	Arachis hypogaea 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	They were all labeled by peanut lectin ( Arachis hypogaea ) and three showed reactivity for S-100 protein .
	manualset3
183534	3	414127	7	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	They were all labeled by peanut lectin ( Arachis hypogaea ) and three showed reactivity for S-100 protein .
	manualset3
183535	4	414127	7	NULL	NULL	0	NULL	reactivity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They were all labeled by peanut lectin ( Arachis hypogaea ) and three showed reactivity for S-100 protein .
	manualset3
183536	5	414127	7	NULL	NULL	0	NULL	S-100 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	They were all labeled by peanut lectin ( Arachis hypogaea ) and three showed reactivity for S-100 protein .
	manualset3
183537	1	414128	7	NULL	NULL	0	NULL	physicochemical data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	They were characterized by physicochemical , elemental , and spectral ( IR , ( 1 ) H-NMR , and Mass ) data .
	manualset3
183538	2	414128	7	NULL	NULL	0	NULL	elemental data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	They were characterized by physicochemical , elemental , and spectral ( IR , ( 1 ) H-NMR , and Mass ) data .
	manualset3
183539	3	414128	7	NULL	NULL	0	NULL	spectral  IR data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	They were characterized by physicochemical , elemental , and spectral ( IR , ( 1 ) H-NMR , and Mass ) data .
	manualset3
183540	4	414128	7	NULL	NULL	0	NULL	( 1 ) H-NMR data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	They were characterized by physicochemical , elemental , and spectral ( IR , ( 1 ) H-NMR , and Mass ) data .
	manualset3
183541	5	414128	7	NULL	NULL	0	NULL	Mass  data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	They were characterized by physicochemical , elemental , and spectral ( IR , ( 1 ) H-NMR , and Mass ) data .
	manualset3
183542	1	414129	7	NULL	NULL	0	NULL	surface-potential distribution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the surface-potential distribution of SOD2 revealed a conserved positively charged electrostatic zone in the proximity of the active site that probably functions in the same way as in Cu/Zn-SODs by facilitating the diffusion of the superoxide anion to the metal ion .
	manualset3
183543	2	414129	7	NULL	NULL	0	NULL	SOD2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the surface-potential distribution of SOD2 revealed a conserved positively charged electrostatic zone in the proximity of the active site that probably functions in the same way as in Cu/Zn-SODs by facilitating the diffusion of the superoxide anion to the metal ion .
	manualset3
183544	3	414129	7	NULL	NULL	0	NULL	conserved positively charged electrostatic zone	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the surface-potential distribution of SOD2 revealed a conserved positively charged electrostatic zone in the proximity of the active site that probably functions in the same way as in Cu/Zn-SODs by facilitating the diffusion of the superoxide anion to the metal ion .
	manualset3
183545	4	414129	7	NULL	NULL	0	NULL	proximity of the active site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the surface-potential distribution of SOD2 revealed a conserved positively charged electrostatic zone in the proximity of the active site that probably functions in the same way as in Cu/Zn-SODs by facilitating the diffusion of the superoxide anion to the metal ion .
	manualset3
183546	5	414129	7	NULL	NULL	0	NULL	 functions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the surface-potential distribution of SOD2 revealed a conserved positively charged electrostatic zone in the proximity of the active site that probably functions in the same way as in Cu/Zn-SODs by facilitating the diffusion of the superoxide anion to the metal ion .
	manualset3
183547	6	414129	7	NULL	NULL	0	NULL	Cu/Zn-SODs	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the surface-potential distribution of SOD2 revealed a conserved positively charged electrostatic zone in the proximity of the active site that probably functions in the same way as in Cu/Zn-SODs by facilitating the diffusion of the superoxide anion to the metal ion .
	manualset3
183548	7	414129	7	NULL	NULL	0	NULL	facilitating	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the surface-potential distribution of SOD2 revealed a conserved positively charged electrostatic zone in the proximity of the active site that probably functions in the same way as in Cu/Zn-SODs by facilitating the diffusion of the superoxide anion to the metal ion .
	manualset3
183549	8	414129	7	NULL	NULL	0	NULL	diffusion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the surface-potential distribution of SOD2 revealed a conserved positively charged electrostatic zone in the proximity of the active site that probably functions in the same way as in Cu/Zn-SODs by facilitating the diffusion of the superoxide anion to the metal ion .
	manualset3
183550	9	414129	7	NULL	NULL	0	NULL	superoxide anion	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the surface-potential distribution of SOD2 revealed a conserved positively charged electrostatic zone in the proximity of the active site that probably functions in the same way as in Cu/Zn-SODs by facilitating the diffusion of the superoxide anion to the metal ion .
	manualset3
183551	10	414129	7	NULL	NULL	0	NULL	metal ion	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the surface-potential distribution of SOD2 revealed a conserved positively charged electrostatic zone in the proximity of the active site that probably functions in the same way as in Cu/Zn-SODs by facilitating the diffusion of the superoxide anion to the metal ion .
	manualset3
183552	1	414130	7	NULL	NULL	0	NULL	delivery catheters	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	They were easily retrieved from within the delivery catheters and the vessels , which is not possible with conventional coils .
	manualset3
183553	2	414130	7	NULL	NULL	0	NULL	vessels	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	They were easily retrieved from within the delivery catheters and the vessels , which is not possible with conventional coils .
	manualset3
183554	3	414130	7	NULL	NULL	0	NULL	conventional coils	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	They were easily retrieved from within the delivery catheters and the vessels , which is not possible with conventional coils .
	manualset3
183559	1	414131	7	NULL	NULL	0	NULL	Bouin 's fluid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	They were fixed in Bouin 's fluid and examined for the presence of alkaline phosphatase by th immunoperoxidase method .
	manualset3
183560	2	414131	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They were fixed in Bouin 's fluid and examined for the presence of alkaline phosphatase by th immunoperoxidase method .
	manualset3
183561	4	414131	7	NULL	NULL	NULL	NULL	th immunoperoxidase method 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	They were fixed in Bouin 's fluid and examined for the presence of alkaline phosphatase by th immunoperoxidase method .
	manualset3
184181	3	414131	7	NULL	NULL	0	NULL	alkaline phosphatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	They were fixed in Bouin 's fluid and examined for the presence of alkaline phosphatase by th immunoperoxidase method .
	manualset3
183562	1	414132	7	NULL	NULL	0	NULL	parts of the circumference	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	They were only present in those parts of the circumference in which the stromal capillaries also revealed structural changes .
	manualset3
183563	2	414132	7	NULL	NULL	0	NULL	stromal capillaries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	They were only present in those parts of the circumference in which the stromal capillaries also revealed structural changes .
	manualset3
183564	3	414132	7	NULL	NULL	0	NULL	structural changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They were only present in those parts of the circumference in which the stromal capillaries also revealed structural changes .
	manualset3
183565	1	414133	7	NULL	NULL	0	NULL	different concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	They were treated with different concentrations ( 0 , 5 , 10 , 25 , 50 , 100 and 200mg/L ) of potassium dichromate solution .
	manualset3
183566	2	414133	7	NULL	NULL	0	NULL	0 mg/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	They were treated with different concentrations ( 0 , 5 , 10 , 25 , 50 , 100 and 200mg/L ) of potassium dichromate solution .
	manualset3
183567	3	414133	7	NULL	NULL	0	NULL	5 mg/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	They were treated with different concentrations ( 0 , 5 , 10 , 25 , 50 , 100 and 200mg/L ) of potassium dichromate solution .
	manualset3
183568	4	414133	7	NULL	NULL	0	NULL	10 mg/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	They were treated with different concentrations ( 0 , 5 , 10 , 25 , 50 , 100 and 200mg/L ) of potassium dichromate solution .
	manualset3
183569	5	414133	7	NULL	NULL	0	NULL	25 mg/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	They were treated with different concentrations ( 0 , 5 , 10 , 25 , 50 , 100 and 200mg/L ) of potassium dichromate solution .
	manualset3
183570	6	414133	7	NULL	NULL	0	NULL	 50 mg/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	They were treated with different concentrations ( 0 , 5 , 10 , 25 , 50 , 100 and 200mg/L ) of potassium dichromate solution .
	manualset3
183571	7	414133	7	NULL	NULL	0	NULL	100 mg/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	They were treated with different concentrations ( 0 , 5 , 10 , 25 , 50 , 100 and 200mg/L ) of potassium dichromate solution .
	manualset3
183572	8	414133	7	NULL	NULL	0	NULL	200mg/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	They were treated with different concentrations ( 0 , 5 , 10 , 25 , 50 , 100 and 200mg/L ) of potassium dichromate solution .
	manualset3
183573	9	414133	7	NULL	NULL	0	NULL	potassium dichromate solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	They were treated with different concentrations ( 0 , 5 , 10 , 25 , 50 , 100 and 200mg/L ) of potassium dichromate solution .
	manualset3
183574	1	414134	7	NULL	NULL	NULL	NULL	Thiazolidinediones	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Thiazolidinediones , represented by troglitazone , are insulin-sensitizing agents with proven efficacy for the treatment of type 2 diabetes .
	manualset3
183575	2	414134	7	NULL	NULL	0	NULL	troglitazone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Thiazolidinediones , represented by troglitazone , are insulin-sensitizing agents with proven efficacy for the treatment of type 2 diabetes .
	manualset3
183576	3	414134	7	NULL	NULL	0	NULL	insulin-sensitizing agents	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Thiazolidinediones , represented by troglitazone , are insulin-sensitizing agents with proven efficacy for the treatment of type 2 diabetes .
	manualset3
183577	4	414134	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Thiazolidinediones , represented by troglitazone , are insulin-sensitizing agents with proven efficacy for the treatment of type 2 diabetes .
	manualset3
183578	5	414134	7	NULL	NULL	0	NULL	type 2 diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Thiazolidinediones , represented by troglitazone , are insulin-sensitizing agents with proven efficacy for the treatment of type 2 diabetes .
	manualset3
183579	1	414135	7	NULL	NULL	0	NULL	Thickening of  trabeculae	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thickening and coalescence of trabeculae were observed , particularly dorsally and medially , causing reduction or elimination of the marrow void spaces .
	manualset3
183580	2	414135	7	NULL	NULL	0	NULL	coalescence of trabeculae	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thickening and coalescence of trabeculae were observed , particularly dorsally and medially , causing reduction or elimination of the marrow void spaces .
	manualset3
183581	3	414135	7	NULL	NULL	0	NULL	reduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thickening and coalescence of trabeculae were observed , particularly dorsally and medially , causing reduction or elimination of the marrow void spaces .
	manualset3
183582	4	414135	7	NULL	NULL	0	NULL	elimination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thickening and coalescence of trabeculae were observed , particularly dorsally and medially , causing reduction or elimination of the marrow void spaces .
	manualset3
183583	5	414135	7	NULL	NULL	0	NULL	marrow void spaces	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Thickening and coalescence of trabeculae were observed , particularly dorsally and medially , causing reduction or elimination of the marrow void spaces .
	manualset3
183584	1	414136	7	NULL	NULL	0	NULL	Thickening	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thickening of the involved optic nerve by less than 1.7 mm is associated with a better prognosis as regards the time and completeness of vision restoration .
	manualset3
183585	2	414136	7	NULL	NULL	0	NULL	optic nerve	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Thickening of the involved optic nerve by less than 1.7 mm is associated with a better prognosis as regards the time and completeness of vision restoration .
	manualset3
183586	3	414136	7	NULL	NULL	0	NULL	1.7 mm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Thickening of the involved optic nerve by less than 1.7 mm is associated with a better prognosis as regards the time and completeness of vision restoration .
	manualset3
183587	4	414136	7	NULL	NULL	0	NULL	better prognosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thickening of the involved optic nerve by less than 1.7 mm is associated with a better prognosis as regards the time and completeness of vision restoration .
	manualset3
183588	5	414136	7	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Thickening of the involved optic nerve by less than 1.7 mm is associated with a better prognosis as regards the time and completeness of vision restoration .
	manualset3
183589	6	414136	7	NULL	NULL	0	NULL	vision restoration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thickening of the involved optic nerve by less than 1.7 mm is associated with a better prognosis as regards the time and completeness of vision restoration .
	manualset3
183590	1	414137	7	NULL	NULL	0	NULL	transcriptional program	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the transcriptional program elicited by caffeine resembled that of rapamycin , a potent inhibitor of the TOR1/2 kinases .
	manualset3
183591	2	414137	7	NULL	NULL	0	NULL	caffeine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the transcriptional program elicited by caffeine resembled that of rapamycin , a potent inhibitor of the TOR1/2 kinases .
	manualset3
183592	3	414137	7	NULL	NULL	0	NULL	rapamycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the transcriptional program elicited by caffeine resembled that of rapamycin , a potent inhibitor of the TOR1/2 kinases .
	manualset3
183593	4	414137	7	NULL	NULL	0	NULL	 inhibitor	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the transcriptional program elicited by caffeine resembled that of rapamycin , a potent inhibitor of the TOR1/2 kinases .
	manualset3
183594	5	414137	7	NULL	NULL	0	NULL	TOR1/2 kinases	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the transcriptional program elicited by caffeine resembled that of rapamycin , a potent inhibitor of the TOR1/2 kinases .
	manualset3
183595	1	414138	7	NULL	NULL	0	NULL	Thinning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Thinning did not alter branch angle , branching density or the relationship between branch size and branch leaf area .
	manualset3
183596	2	414138	7	NULL	NULL	0	NULL	 branch angle	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thinning did not alter branch angle , branching density or the relationship between branch size and branch leaf area .
	manualset3
183597	3	414138	7	NULL	NULL	0	NULL	branching density	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thinning did not alter branch angle , branching density or the relationship between branch size and branch leaf area .
	manualset3
183598	4	414138	7	NULL	NULL	0	NULL	 relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Thinning did not alter branch angle , branching density or the relationship between branch size and branch leaf area .
	manualset3
183599	5	414138	7	NULL	NULL	0	NULL	branch size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thinning did not alter branch angle , branching density or the relationship between branch size and branch leaf area .
	manualset3
183600	6	414138	7	NULL	NULL	0	NULL	branch leaf area	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thinning did not alter branch angle , branching density or the relationship between branch size and branch leaf area .
	manualset3
183601	1	414139	7	NULL	NULL	0	NULL	Thioacetamide-induced acute liver failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thioacetamide-induced acute liver failure in rats resulted in significant decreases in the Kir4 .1 mRNA and protein contents of cerebral cortex , whereas expression of Kir2 .1 and NKCC1 remained unaltered .
	manualset3
183602	2	414139	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Thioacetamide-induced acute liver failure in rats resulted in significant decreases in the Kir4 .1 mRNA and protein contents of cerebral cortex , whereas expression of Kir2 .1 and NKCC1 remained unaltered .
	manualset3
183603	3	414139	7	NULL	NULL	0	NULL	Kir4 .1 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Thioacetamide-induced acute liver failure in rats resulted in significant decreases in the Kir4 .1 mRNA and protein contents of cerebral cortex , whereas expression of Kir2 .1 and NKCC1 remained unaltered .
	manualset3
183604	4	414139	7	NULL	NULL	0	NULL	Kir4 .1 protein content	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thioacetamide-induced acute liver failure in rats resulted in significant decreases in the Kir4 .1 mRNA and protein contents of cerebral cortex , whereas expression of Kir2 .1 and NKCC1 remained unaltered .
	manualset3
183605	5	414139	7	NULL	NULL	0	NULL	 cerebral cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Thioacetamide-induced acute liver failure in rats resulted in significant decreases in the Kir4 .1 mRNA and protein contents of cerebral cortex , whereas expression of Kir2 .1 and NKCC1 remained unaltered .
	manualset3
183606	6	414139	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thioacetamide-induced acute liver failure in rats resulted in significant decreases in the Kir4 .1 mRNA and protein contents of cerebral cortex , whereas expression of Kir2 .1 and NKCC1 remained unaltered .
	manualset3
183607	7	414139	7	NULL	NULL	0	NULL	Kir2 .1	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thioacetamide-induced acute liver failure in rats resulted in significant decreases in the Kir4 .1 mRNA and protein contents of cerebral cortex , whereas expression of Kir2 .1 and NKCC1 remained unaltered .
	manualset3
183608	8	414139	7	NULL	NULL	0	NULL	NKCC1 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thioacetamide-induced acute liver failure in rats resulted in significant decreases in the Kir4 .1 mRNA and protein contents of cerebral cortex , whereas expression of Kir2 .1 and NKCC1 remained unaltered .
	manualset3
183609	1	414140	7	NULL	NULL	0	NULL	Thioglycollate injection	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Thioglycollate injection ( 1 ml ip ) was used as an inflammatory challenge and to partially activate macrophages for cytotoxicity .
	manualset3
183610	2	414140	7	NULL	NULL	0	NULL	1 ml ip	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Thioglycollate injection ( 1 ml ip ) was used as an inflammatory challenge and to partially activate macrophages for cytotoxicity .
	manualset3
183611	3	414140	7	NULL	NULL	0	NULL	inflammatory challenge	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thioglycollate injection ( 1 ml ip ) was used as an inflammatory challenge and to partially activate macrophages for cytotoxicity .
	manualset3
183612	4	414140	7	NULL	NULL	0	NULL	macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Thioglycollate injection ( 1 ml ip ) was used as an inflammatory challenge and to partially activate macrophages for cytotoxicity .
	manualset3
183613	5	414140	7	NULL	NULL	0	NULL	cytotoxicity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thioglycollate injection ( 1 ml ip ) was used as an inflammatory challenge and to partially activate macrophages for cytotoxicity .
	manualset3
183614	1	414141	7	NULL	NULL	0	NULL	Thioureas	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Thioureas differentially induce rat hepatic microsomal epoxide hydrolase and rGSTA2 irrespective of their oxygen radical scavenging effect : effects on toxicant-induced liver injury .
	manualset3
183615	2	414141	7	NULL	NULL	0	NULL	rat hepatic microsomal epoxide hydrolase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thioureas differentially induce rat hepatic microsomal epoxide hydrolase and rGSTA2 irrespective of their oxygen radical scavenging effect : effects on toxicant-induced liver injury .
	manualset3
183616	3	414141	7	NULL	NULL	0	NULL	rGSTA2	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thioureas differentially induce rat hepatic microsomal epoxide hydrolase and rGSTA2 irrespective of their oxygen radical scavenging effect : effects on toxicant-induced liver injury .
	manualset3
183617	4	414141	7	NULL	NULL	NULL	NULL	oxygen radical scavenging effect	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Thioureas differentially induce rat hepatic microsomal epoxide hydrolase and rGSTA2 irrespective of their oxygen radical scavenging effect : effects on toxicant-induced liver injury .
	manualset3
183618	5	414141	7	NULL	NULL	0	NULL	toxicant-induced liver injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thioureas differentially induce rat hepatic microsomal epoxide hydrolase and rGSTA2 irrespective of their oxygen radical scavenging effect : effects on toxicant-induced liver injury .
	manualset3
183619	1	414142	7	NULL	NULL	0	NULL	Third-generation aromatase inhibitors ( AIs )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Third-generation aromatase inhibitors ( AIs ) are replacing tamoxifen as adjuvant therapy in postmenopausal women with hormone-sensitive breast cancer due to their superiority shown in several recent head-to-head trials .
	manualset3
183620	2	414142	7	NULL	NULL	0	NULL	tamoxifen	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Third-generation aromatase inhibitors ( AIs ) are replacing tamoxifen as adjuvant therapy in postmenopausal women with hormone-sensitive breast cancer due to their superiority shown in several recent head-to-head trials .
	manualset3
183621	3	414142	7	NULL	NULL	0	NULL	adjuvant therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Third-generation aromatase inhibitors ( AIs ) are replacing tamoxifen as adjuvant therapy in postmenopausal women with hormone-sensitive breast cancer due to their superiority shown in several recent head-to-head trials .
	manualset3
183622	4	414142	7	NULL	NULL	0	NULL	postmenopausal women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Third-generation aromatase inhibitors ( AIs ) are replacing tamoxifen as adjuvant therapy in postmenopausal women with hormone-sensitive breast cancer due to their superiority shown in several recent head-to-head trials .
	manualset3
183623	5	414142	7	NULL	NULL	0	NULL	hormone-sensitive breast cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Third-generation aromatase inhibitors ( AIs ) are replacing tamoxifen as adjuvant therapy in postmenopausal women with hormone-sensitive breast cancer due to their superiority shown in several recent head-to-head trials .
	manualset3
183624	6	414142	7	NULL	NULL	0	NULL	head-to-head trials	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Third-generation aromatase inhibitors ( AIs ) are replacing tamoxifen as adjuvant therapy in postmenopausal women with hormone-sensitive breast cancer due to their superiority shown in several recent head-to-head trials .
	manualset3
183625	1	414143	7	NULL	NULL	0	NULL	Third party reimbursement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Third party reimbursement good for nurses and patients .
	manualset3
183626	2	414143	7	NULL	NULL	0	NULL	nurses	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Third party reimbursement good for nurses and patients .
	manualset3
183627	3	414143	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Third party reimbursement good for nurses and patients .
	manualset3
183628	1	414144	7	NULL	NULL	0	NULL	Third trimester	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Third trimester intra uterine death following spontaneous hemoperitoneum .
	manualset3
183629	2	414144	7	NULL	NULL	0	NULL	intra uterine death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Third trimester intra uterine death following spontaneous hemoperitoneum .
	manualset3
183630	3	414144	7	NULL	NULL	0	NULL	spontaneous hemoperitoneum	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Third trimester intra uterine death following spontaneous hemoperitoneum .
	manualset3
183631	1	414145	7	NULL	NULL	0	NULL	CD8 ( + ) T cell response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Third , it seemed that the overall CD8 ( + ) T cell response was augmented with increasing severity of disease , while the LCMV-specific CD4 ( + ) T cell response magnitude was highly variable between the three different donors .
	manualset3
183632	2	414145	7	NULL	NULL	0	NULL	severity of disease	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Third , it seemed that the overall CD8 ( + ) T cell response was augmented with increasing severity of disease , while the LCMV-specific CD4 ( + ) T cell response magnitude was highly variable between the three different donors .
	manualset3
183633	3	414145	7	NULL	NULL	0	NULL	LCMV-specific CD4 ( + ) T cell response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Third , it seemed that the overall CD8 ( + ) T cell response was augmented with increasing severity of disease , while the LCMV-specific CD4 ( + ) T cell response magnitude was highly variable between the three different donors .
	manualset3
183634	4	414145	7	NULL	NULL	0	NULL	variable 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Third , it seemed that the overall CD8 ( + ) T cell response was augmented with increasing severity of disease , while the LCMV-specific CD4 ( + ) T cell response magnitude was highly variable between the three different donors .
	manualset3
183635	5	414145	7	NULL	NULL	0	NULL	three different donors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Third , it seemed that the overall CD8 ( + ) T cell response was augmented with increasing severity of disease , while the LCMV-specific CD4 ( + ) T cell response magnitude was highly variable between the three different donors .
	manualset3
183636	1	414146	7	NULL	NULL	0	NULL	search	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Third , the search for an inexpensive , rapid , sensitive , and specific TB diagnostic that is able to replace smear and delayed mycobacterial culture has yielded promising results .
	manualset3
183637	2	414146	7	NULL	NULL	0	NULL	specific TB diagnostic	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Third , the search for an inexpensive , rapid , sensitive , and specific TB diagnostic that is able to replace smear and delayed mycobacterial culture has yielded promising results .
	manualset3
183638	3	414146	7	NULL	NULL	0	NULL	smear	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Third , the search for an inexpensive , rapid , sensitive , and specific TB diagnostic that is able to replace smear and delayed mycobacterial culture has yielded promising results .
	manualset3
183639	4	414146	7	NULL	NULL	0	NULL	delayed mycobacterial culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Third , the search for an inexpensive , rapid , sensitive , and specific TB diagnostic that is able to replace smear and delayed mycobacterial culture has yielded promising results .
	manualset3
183640	5	414146	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Third , the search for an inexpensive , rapid , sensitive , and specific TB diagnostic that is able to replace smear and delayed mycobacterial culture has yielded promising results .
	manualset3
183641	1	414147	7	NULL	NULL	0	NULL	diabetes-dependent differences	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Third , we demonstrate marked diabetes-dependent differences in the amount of redox active iron present in the plasma of mice genetically modified expressing the Hp 2 allele as compared with the Hp 1 allele .
	manualset3
183642	2	414147	7	NULL	NULL	0	NULL	amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Third , we demonstrate marked diabetes-dependent differences in the amount of redox active iron present in the plasma of mice genetically modified expressing the Hp 2 allele as compared with the Hp 1 allele .
	manualset3
183643	3	414147	7	NULL	NULL	0	NULL	redox active iron	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Third , we demonstrate marked diabetes-dependent differences in the amount of redox active iron present in the plasma of mice genetically modified expressing the Hp 2 allele as compared with the Hp 1 allele .
	manualset3
183644	4	414147	7	NULL	NULL	0	NULL	plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Third , we demonstrate marked diabetes-dependent differences in the amount of redox active iron present in the plasma of mice genetically modified expressing the Hp 2 allele as compared with the Hp 1 allele .
	manualset3
183645	5	414147	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Third , we demonstrate marked diabetes-dependent differences in the amount of redox active iron present in the plasma of mice genetically modified expressing the Hp 2 allele as compared with the Hp 1 allele .
	manualset3
183646	6	414147	7	NULL	NULL	0	NULL	Hp 2 allele	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Third , we demonstrate marked diabetes-dependent differences in the amount of redox active iron present in the plasma of mice genetically modified expressing the Hp 2 allele as compared with the Hp 1 allele .
	manualset3
183647	7	414147	7	NULL	NULL	0	NULL	Hp 1 allele	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Third , we demonstrate marked diabetes-dependent differences in the amount of redox active iron present in the plasma of mice genetically modified expressing the Hp 2 allele as compared with the Hp 1 allele .
	manualset3
183648	1	414148	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the treatment and prognosis for mucinous cystadenocarcinoma of the appendix are noted .
	manualset3
183649	2	414148	7	NULL	NULL	0	NULL	prognosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the treatment and prognosis for mucinous cystadenocarcinoma of the appendix are noted .
	manualset3
183650	3	414148	7	NULL	NULL	0	NULL	mucinous cystadenocarcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the treatment and prognosis for mucinous cystadenocarcinoma of the appendix are noted .
	manualset3
183651	4	414148	7	NULL	NULL	0	NULL	appendix	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the treatment and prognosis for mucinous cystadenocarcinoma of the appendix are noted .
	manualset3
183652	1	414149	7	NULL	NULL	0	NULL	Thirteen individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen individuals living in nonendemic areas who had negative serology were used as a negative control group : 100 % had negative PCR results .
	manualset3
183653	2	414149	7	NULL	NULL	0	NULL	nonendemic areas	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen individuals living in nonendemic areas who had negative serology were used as a negative control group : 100 % had negative PCR results .
	manualset3
183654	3	414149	7	NULL	NULL	0	NULL	negative serology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen individuals living in nonendemic areas who had negative serology were used as a negative control group : 100 % had negative PCR results .
	manualset3
183655	4	414149	7	NULL	NULL	0	NULL	 negative control group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen individuals living in nonendemic areas who had negative serology were used as a negative control group : 100 % had negative PCR results .
	manualset3
183656	5	414149	7	NULL	NULL	0	NULL	100 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen individuals living in nonendemic areas who had negative serology were used as a negative control group : 100 % had negative PCR results .
	manualset3
183657	6	414149	7	NULL	NULL	0	NULL	negative PCR results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen individuals living in nonendemic areas who had negative serology were used as a negative control group : 100 % had negative PCR results .
	manualset3
183658	1	414150	7	NULL	NULL	0	NULL	Thirteen infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen infants and 2 children with Herpes simplex encephalitis are reported and the authors emphasize the diagnostic value of several investigations : the neurological examination ( fits followed by early motor deficit on the same side and coma ) , the EEG ( periodicity and asymmetry of the trace ) , the CT scan ( hypodensity in the frontotemporal areas ) , the level of the Interferon alpha in blood and cerebrospinal fluid , the electrophoretic pattern of cerebrospinal fluid proteins and the comparative study of cerebrospinal fluid/serum antibodies towards several viral antigens .
	manualset3
183659	2	414150	7	NULL	NULL	0	NULL	2 children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen infants and 2 children with Herpes simplex encephalitis are reported and the authors emphasize the diagnostic value of several investigations : the neurological examination ( fits followed by early motor deficit on the same side and coma ) , the EEG ( periodicity and asymmetry of the trace ) , the CT scan ( hypodensity in the frontotemporal areas ) , the level of the Interferon alpha in blood and cerebrospinal fluid , the electrophoretic pattern of cerebrospinal fluid proteins and the comparative study of cerebrospinal fluid/serum antibodies towards several viral antigens .
	manualset3
183660	3	414150	7	NULL	NULL	0	NULL	Herpes simplex encephalitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen infants and 2 children with Herpes simplex encephalitis are reported and the authors emphasize the diagnostic value of several investigations : the neurological examination ( fits followed by early motor deficit on the same side and coma ) , the EEG ( periodicity and asymmetry of the trace ) , the CT scan ( hypodensity in the frontotemporal areas ) , the level of the Interferon alpha in blood and cerebrospinal fluid , the electrophoretic pattern of cerebrospinal fluid proteins and the comparative study of cerebrospinal fluid/serum antibodies towards several viral antigens .
	manualset3
183661	4	414150	7	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen infants and 2 children with Herpes simplex encephalitis are reported and the authors emphasize the diagnostic value of several investigations : the neurological examination ( fits followed by early motor deficit on the same side and coma ) , the EEG ( periodicity and asymmetry of the trace ) , the CT scan ( hypodensity in the frontotemporal areas ) , the level of the Interferon alpha in blood and cerebrospinal fluid , the electrophoretic pattern of cerebrospinal fluid proteins and the comparative study of cerebrospinal fluid/serum antibodies towards several viral antigens .
	manualset3
183662	5	414150	7	NULL	NULL	0	NULL	diagnostic value	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen infants and 2 children with Herpes simplex encephalitis are reported and the authors emphasize the diagnostic value of several investigations : the neurological examination ( fits followed by early motor deficit on the same side and coma ) , the EEG ( periodicity and asymmetry of the trace ) , the CT scan ( hypodensity in the frontotemporal areas ) , the level of the Interferon alpha in blood and cerebrospinal fluid , the electrophoretic pattern of cerebrospinal fluid proteins and the comparative study of cerebrospinal fluid/serum antibodies towards several viral antigens .
	manualset3
183663	6	414150	7	NULL	NULL	0	NULL	investigations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen infants and 2 children with Herpes simplex encephalitis are reported and the authors emphasize the diagnostic value of several investigations : the neurological examination ( fits followed by early motor deficit on the same side and coma ) , the EEG ( periodicity and asymmetry of the trace ) , the CT scan ( hypodensity in the frontotemporal areas ) , the level of the Interferon alpha in blood and cerebrospinal fluid , the electrophoretic pattern of cerebrospinal fluid proteins and the comparative study of cerebrospinal fluid/serum antibodies towards several viral antigens .
	manualset3
183664	7	414150	7	NULL	NULL	NULL	NULL	neurological examination 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Thirteen infants and 2 children with Herpes simplex encephalitis are reported and the authors emphasize the diagnostic value of several investigations : the neurological examination ( fits followed by early motor deficit on the same side and coma ) , the EEG ( periodicity and asymmetry of the trace ) , the CT scan ( hypodensity in the frontotemporal areas ) , the level of the Interferon alpha in blood and cerebrospinal fluid , the electrophoretic pattern of cerebrospinal fluid proteins and the comparative study of cerebrospinal fluid/serum antibodies towards several viral antigens .
	manualset3
183665	8	414150	7	NULL	NULL	0	NULL	 fits 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen infants and 2 children with Herpes simplex encephalitis are reported and the authors emphasize the diagnostic value of several investigations : the neurological examination ( fits followed by early motor deficit on the same side and coma ) , the EEG ( periodicity and asymmetry of the trace ) , the CT scan ( hypodensity in the frontotemporal areas ) , the level of the Interferon alpha in blood and cerebrospinal fluid , the electrophoretic pattern of cerebrospinal fluid proteins and the comparative study of cerebrospinal fluid/serum antibodies towards several viral antigens .
	manualset3
183666	9	414150	7	NULL	NULL	0	NULL	 early motor deficit	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen infants and 2 children with Herpes simplex encephalitis are reported and the authors emphasize the diagnostic value of several investigations : the neurological examination ( fits followed by early motor deficit on the same side and coma ) , the EEG ( periodicity and asymmetry of the trace ) , the CT scan ( hypodensity in the frontotemporal areas ) , the level of the Interferon alpha in blood and cerebrospinal fluid , the electrophoretic pattern of cerebrospinal fluid proteins and the comparative study of cerebrospinal fluid/serum antibodies towards several viral antigens .
	manualset3
183667	10	414150	7	NULL	NULL	0	NULL	same side	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen infants and 2 children with Herpes simplex encephalitis are reported and the authors emphasize the diagnostic value of several investigations : the neurological examination ( fits followed by early motor deficit on the same side and coma ) , the EEG ( periodicity and asymmetry of the trace ) , the CT scan ( hypodensity in the frontotemporal areas ) , the level of the Interferon alpha in blood and cerebrospinal fluid , the electrophoretic pattern of cerebrospinal fluid proteins and the comparative study of cerebrospinal fluid/serum antibodies towards several viral antigens .
	manualset3
183668	11	414150	7	NULL	NULL	0	NULL	coma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen infants and 2 children with Herpes simplex encephalitis are reported and the authors emphasize the diagnostic value of several investigations : the neurological examination ( fits followed by early motor deficit on the same side and coma ) , the EEG ( periodicity and asymmetry of the trace ) , the CT scan ( hypodensity in the frontotemporal areas ) , the level of the Interferon alpha in blood and cerebrospinal fluid , the electrophoretic pattern of cerebrospinal fluid proteins and the comparative study of cerebrospinal fluid/serum antibodies towards several viral antigens .
	manualset3
183669	12	414150	7	NULL	NULL	0	NULL	EEG	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen infants and 2 children with Herpes simplex encephalitis are reported and the authors emphasize the diagnostic value of several investigations : the neurological examination ( fits followed by early motor deficit on the same side and coma ) , the EEG ( periodicity and asymmetry of the trace ) , the CT scan ( hypodensity in the frontotemporal areas ) , the level of the Interferon alpha in blood and cerebrospinal fluid , the electrophoretic pattern of cerebrospinal fluid proteins and the comparative study of cerebrospinal fluid/serum antibodies towards several viral antigens .
	manualset3
183670	13	414150	7	NULL	NULL	0	NULL	periodicity	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen infants and 2 children with Herpes simplex encephalitis are reported and the authors emphasize the diagnostic value of several investigations : the neurological examination ( fits followed by early motor deficit on the same side and coma ) , the EEG ( periodicity and asymmetry of the trace ) , the CT scan ( hypodensity in the frontotemporal areas ) , the level of the Interferon alpha in blood and cerebrospinal fluid , the electrophoretic pattern of cerebrospinal fluid proteins and the comparative study of cerebrospinal fluid/serum antibodies towards several viral antigens .
	manualset3
183671	14	414150	7	NULL	NULL	0	NULL	asymmetry of the trace	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen infants and 2 children with Herpes simplex encephalitis are reported and the authors emphasize the diagnostic value of several investigations : the neurological examination ( fits followed by early motor deficit on the same side and coma ) , the EEG ( periodicity and asymmetry of the trace ) , the CT scan ( hypodensity in the frontotemporal areas ) , the level of the Interferon alpha in blood and cerebrospinal fluid , the electrophoretic pattern of cerebrospinal fluid proteins and the comparative study of cerebrospinal fluid/serum antibodies towards several viral antigens .
	manualset3
183672	15	414150	7	NULL	NULL	0	NULL	CT scan	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen infants and 2 children with Herpes simplex encephalitis are reported and the authors emphasize the diagnostic value of several investigations : the neurological examination ( fits followed by early motor deficit on the same side and coma ) , the EEG ( periodicity and asymmetry of the trace ) , the CT scan ( hypodensity in the frontotemporal areas ) , the level of the Interferon alpha in blood and cerebrospinal fluid , the electrophoretic pattern of cerebrospinal fluid proteins and the comparative study of cerebrospinal fluid/serum antibodies towards several viral antigens .
	manualset3
183673	16	414150	7	NULL	NULL	0	NULL	hypodensity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen infants and 2 children with Herpes simplex encephalitis are reported and the authors emphasize the diagnostic value of several investigations : the neurological examination ( fits followed by early motor deficit on the same side and coma ) , the EEG ( periodicity and asymmetry of the trace ) , the CT scan ( hypodensity in the frontotemporal areas ) , the level of the Interferon alpha in blood and cerebrospinal fluid , the electrophoretic pattern of cerebrospinal fluid proteins and the comparative study of cerebrospinal fluid/serum antibodies towards several viral antigens .
	manualset3
183674	17	414150	7	NULL	NULL	0	NULL	frontotemporal areas 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen infants and 2 children with Herpes simplex encephalitis are reported and the authors emphasize the diagnostic value of several investigations : the neurological examination ( fits followed by early motor deficit on the same side and coma ) , the EEG ( periodicity and asymmetry of the trace ) , the CT scan ( hypodensity in the frontotemporal areas ) , the level of the Interferon alpha in blood and cerebrospinal fluid , the electrophoretic pattern of cerebrospinal fluid proteins and the comparative study of cerebrospinal fluid/serum antibodies towards several viral antigens .
	manualset3
183675	18	414150	7	NULL	NULL	0	NULL	 level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen infants and 2 children with Herpes simplex encephalitis are reported and the authors emphasize the diagnostic value of several investigations : the neurological examination ( fits followed by early motor deficit on the same side and coma ) , the EEG ( periodicity and asymmetry of the trace ) , the CT scan ( hypodensity in the frontotemporal areas ) , the level of the Interferon alpha in blood and cerebrospinal fluid , the electrophoretic pattern of cerebrospinal fluid proteins and the comparative study of cerebrospinal fluid/serum antibodies towards several viral antigens .
	manualset3
183676	19	414150	7	NULL	NULL	0	NULL	Interferon alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen infants and 2 children with Herpes simplex encephalitis are reported and the authors emphasize the diagnostic value of several investigations : the neurological examination ( fits followed by early motor deficit on the same side and coma ) , the EEG ( periodicity and asymmetry of the trace ) , the CT scan ( hypodensity in the frontotemporal areas ) , the level of the Interferon alpha in blood and cerebrospinal fluid , the electrophoretic pattern of cerebrospinal fluid proteins and the comparative study of cerebrospinal fluid/serum antibodies towards several viral antigens .
	manualset3
183677	20	414150	7	NULL	NULL	0	NULL	blood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen infants and 2 children with Herpes simplex encephalitis are reported and the authors emphasize the diagnostic value of several investigations : the neurological examination ( fits followed by early motor deficit on the same side and coma ) , the EEG ( periodicity and asymmetry of the trace ) , the CT scan ( hypodensity in the frontotemporal areas ) , the level of the Interferon alpha in blood and cerebrospinal fluid , the electrophoretic pattern of cerebrospinal fluid proteins and the comparative study of cerebrospinal fluid/serum antibodies towards several viral antigens .
	manualset3
183678	21	414150	7	NULL	NULL	0	NULL	cerebrospinal fluid 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen infants and 2 children with Herpes simplex encephalitis are reported and the authors emphasize the diagnostic value of several investigations : the neurological examination ( fits followed by early motor deficit on the same side and coma ) , the EEG ( periodicity and asymmetry of the trace ) , the CT scan ( hypodensity in the frontotemporal areas ) , the level of the Interferon alpha in blood and cerebrospinal fluid , the electrophoretic pattern of cerebrospinal fluid proteins and the comparative study of cerebrospinal fluid/serum antibodies towards several viral antigens .
	manualset3
183679	22	414150	7	NULL	NULL	0	NULL	electrophoretic pattern	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen infants and 2 children with Herpes simplex encephalitis are reported and the authors emphasize the diagnostic value of several investigations : the neurological examination ( fits followed by early motor deficit on the same side and coma ) , the EEG ( periodicity and asymmetry of the trace ) , the CT scan ( hypodensity in the frontotemporal areas ) , the level of the Interferon alpha in blood and cerebrospinal fluid , the electrophoretic pattern of cerebrospinal fluid proteins and the comparative study of cerebrospinal fluid/serum antibodies towards several viral antigens .
	manualset3
183680	23	414150	7	NULL	NULL	0	NULL	cerebrospinal fluid proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen infants and 2 children with Herpes simplex encephalitis are reported and the authors emphasize the diagnostic value of several investigations : the neurological examination ( fits followed by early motor deficit on the same side and coma ) , the EEG ( periodicity and asymmetry of the trace ) , the CT scan ( hypodensity in the frontotemporal areas ) , the level of the Interferon alpha in blood and cerebrospinal fluid , the electrophoretic pattern of cerebrospinal fluid proteins and the comparative study of cerebrospinal fluid/serum antibodies towards several viral antigens .
	manualset3
183681	24	414150	7	NULL	NULL	0	NULL	comparative study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen infants and 2 children with Herpes simplex encephalitis are reported and the authors emphasize the diagnostic value of several investigations : the neurological examination ( fits followed by early motor deficit on the same side and coma ) , the EEG ( periodicity and asymmetry of the trace ) , the CT scan ( hypodensity in the frontotemporal areas ) , the level of the Interferon alpha in blood and cerebrospinal fluid , the electrophoretic pattern of cerebrospinal fluid proteins and the comparative study of cerebrospinal fluid/serum antibodies towards several viral antigens .
	manualset3
183682	25	414150	7	NULL	NULL	0	NULL	cerebrospinal fluid/serum antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen infants and 2 children with Herpes simplex encephalitis are reported and the authors emphasize the diagnostic value of several investigations : the neurological examination ( fits followed by early motor deficit on the same side and coma ) , the EEG ( periodicity and asymmetry of the trace ) , the CT scan ( hypodensity in the frontotemporal areas ) , the level of the Interferon alpha in blood and cerebrospinal fluid , the electrophoretic pattern of cerebrospinal fluid proteins and the comparative study of cerebrospinal fluid/serum antibodies towards several viral antigens .
	manualset3
183683	26	414150	7	NULL	NULL	0	NULL	 viral antigens	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen infants and 2 children with Herpes simplex encephalitis are reported and the authors emphasize the diagnostic value of several investigations : the neurological examination ( fits followed by early motor deficit on the same side and coma ) , the EEG ( periodicity and asymmetry of the trace ) , the CT scan ( hypodensity in the frontotemporal areas ) , the level of the Interferon alpha in blood and cerebrospinal fluid , the electrophoretic pattern of cerebrospinal fluid proteins and the comparative study of cerebrospinal fluid/serum antibodies towards several viral antigens .
	manualset3
183684	1	414151	7	NULL	NULL	0	NULL	Thirteen	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen of these relapsed , with a median time to relapse from the start of treatment of 5 months ( range 3-14 ) .
	manualset3
183685	2	414151	7	NULL	NULL	0	NULL	median time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen of these relapsed , with a median time to relapse from the start of treatment of 5 months ( range 3-14 ) .
	manualset3
183686	3	414151	7	NULL	NULL	0	NULL	start of treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen of these relapsed , with a median time to relapse from the start of treatment of 5 months ( range 3-14 ) .
	manualset3
183687	4	414151	7	NULL	NULL	0	NULL	 5 months 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen of these relapsed , with a median time to relapse from the start of treatment of 5 months ( range 3-14 ) .
	manualset3
183688	5	414151	7	NULL	NULL	0	NULL	range 3-14	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen of these relapsed , with a median time to relapse from the start of treatment of 5 months ( range 3-14 ) .
	manualset3
183689	1	414152	7	NULL	NULL	0	NULL	Thirteen 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen of these were squamous cell carcinomas , 3 were adenocarcinomas and 1 small cell lung carcinoma .
	manualset3
183690	2	414152	7	NULL	NULL	0	NULL	squamous cell carcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen of these were squamous cell carcinomas , 3 were adenocarcinomas and 1 small cell lung carcinoma .
	manualset3
183691	3	414152	7	NULL	NULL	0	NULL	3	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen of these were squamous cell carcinomas , 3 were adenocarcinomas and 1 small cell lung carcinoma .
	manualset3
183692	4	414152	7	NULL	NULL	0	NULL	adenocarcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen of these were squamous cell carcinomas , 3 were adenocarcinomas and 1 small cell lung carcinoma .
	manualset3
183693	5	414152	7	NULL	NULL	0	NULL	1	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen of these were squamous cell carcinomas , 3 were adenocarcinomas and 1 small cell lung carcinoma .
	manualset3
183694	6	414152	7	NULL	NULL	0	NULL	small cell lung carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen of these were squamous cell carcinomas , 3 were adenocarcinomas and 1 small cell lung carcinoma .
	manualset3
183695	1	414153	7	NULL	NULL	0	NULL	Thirteen patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen patients were totally relieved of pain , and three had mild pain .
	manualset3
183696	2	414153	7	NULL	NULL	0	NULL	pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen patients were totally relieved of pain , and three had mild pain .
	manualset3
183697	3	414153	7	NULL	NULL	0	NULL	three 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen patients were totally relieved of pain , and three had mild pain .
	manualset3
183698	4	414153	7	NULL	NULL	0	NULL	mild pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirteen patients were totally relieved of pain , and three had mild pain .
	manualset3
183699	1	414154	7	NULL	NULL	0	NULL	Thirty-eight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-eight of the 64 patients with adenomyomatosis had black pigment gallstones , alone ( n = 22 ) or in association with single ( n = 12 ) or multiple ( n = 4 ) cholesterol gallstones in the same gallbladder .
	manualset3
183700	2	414154	7	NULL	NULL	NULL	NULL	64 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Thirty-eight of the 64 patients with adenomyomatosis had black pigment gallstones , alone ( n = 22 ) or in association with single ( n = 12 ) or multiple ( n = 4 ) cholesterol gallstones in the same gallbladder .
	manualset3
183701	3	414154	7	NULL	NULL	0	NULL	adenomyomatosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-eight of the 64 patients with adenomyomatosis had black pigment gallstones , alone ( n = 22 ) or in association with single ( n = 12 ) or multiple ( n = 4 ) cholesterol gallstones in the same gallbladder .
	manualset3
183702	4	414154	7	NULL	NULL	0	NULL	black pigment gallstones 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-eight of the 64 patients with adenomyomatosis had black pigment gallstones , alone ( n = 22 ) or in association with single ( n = 12 ) or multiple ( n = 4 ) cholesterol gallstones in the same gallbladder .
	manualset3
183703	5	414154	7	NULL	NULL	0	NULL	n=22	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-eight of the 64 patients with adenomyomatosis had black pigment gallstones , alone ( n = 22 ) or in association with single ( n = 12 ) or multiple ( n = 4 ) cholesterol gallstones in the same gallbladder .
	manualset3
183704	6	414154	7	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-eight of the 64 patients with adenomyomatosis had black pigment gallstones , alone ( n = 22 ) or in association with single ( n = 12 ) or multiple ( n = 4 ) cholesterol gallstones in the same gallbladder .
	manualset3
183705	7	414154	7	NULL	NULL	0	NULL	single	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-eight of the 64 patients with adenomyomatosis had black pigment gallstones , alone ( n = 22 ) or in association with single ( n = 12 ) or multiple ( n = 4 ) cholesterol gallstones in the same gallbladder .
	manualset3
183706	8	414154	7	NULL	NULL	0	NULL	n=12	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-eight of the 64 patients with adenomyomatosis had black pigment gallstones , alone ( n = 22 ) or in association with single ( n = 12 ) or multiple ( n = 4 ) cholesterol gallstones in the same gallbladder .
	manualset3
183707	9	414154	7	NULL	NULL	0	NULL	multiple	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-eight of the 64 patients with adenomyomatosis had black pigment gallstones , alone ( n = 22 ) or in association with single ( n = 12 ) or multiple ( n = 4 ) cholesterol gallstones in the same gallbladder .
	manualset3
183708	10	414154	7	NULL	NULL	0	NULL	n=4	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-eight of the 64 patients with adenomyomatosis had black pigment gallstones , alone ( n = 22 ) or in association with single ( n = 12 ) or multiple ( n = 4 ) cholesterol gallstones in the same gallbladder .
	manualset3
183709	11	414154	7	NULL	NULL	0	NULL	cholesterol gallstones	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-eight of the 64 patients with adenomyomatosis had black pigment gallstones , alone ( n = 22 ) or in association with single ( n = 12 ) or multiple ( n = 4 ) cholesterol gallstones in the same gallbladder .
	manualset3
183710	12	414154	7	NULL	NULL	0	NULL	gallbladder	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-eight of the 64 patients with adenomyomatosis had black pigment gallstones , alone ( n = 22 ) or in association with single ( n = 12 ) or multiple ( n = 4 ) cholesterol gallstones in the same gallbladder .
	manualset3
183711	1	414155	7	NULL	NULL	0	NULL	Thirty-eight patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-eight patients were alive without serious complications , and seven had died of unrelated causes .
	manualset3
183712	2	414155	7	NULL	NULL	0	NULL	serious complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-eight patients were alive without serious complications , and seven had died of unrelated causes .
	manualset3
183713	3	414155	7	NULL	NULL	NULL	NULL	seven	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Thirty-eight patients were alive without serious complications , and seven had died of unrelated causes .
	manualset3
185576	4	414155	7	NULL	NULL	0	NULL	unrelated causes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-eight patients were alive without serious complications , and seven had died of unrelated causes .
	manualset3
183714	1	414156	7	NULL	NULL	0	NULL	Thirty-five consecutive days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-five consecutive days of propranolol treatment significantly lowered blood pressure in the older established spontaneous hypertensive rat and prevented the increases from occurring in the younger , developing hypertensive rat .
	manualset3
183715	2	414156	7	NULL	NULL	0	NULL	propranolol treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-five consecutive days of propranolol treatment significantly lowered blood pressure in the older established spontaneous hypertensive rat and prevented the increases from occurring in the younger , developing hypertensive rat .
	manualset3
183716	3	414156	7	NULL	NULL	0	NULL	blood pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-five consecutive days of propranolol treatment significantly lowered blood pressure in the older established spontaneous hypertensive rat and prevented the increases from occurring in the younger , developing hypertensive rat .
	manualset3
183717	4	414156	7	NULL	NULL	0	NULL	 hypertensive rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-five consecutive days of propranolol treatment significantly lowered blood pressure in the older established spontaneous hypertensive rat and prevented the increases from occurring in the younger , developing hypertensive rat .
	manualset3
183718	5	414156	7	NULL	NULL	0	NULL	hypertensive rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-five consecutive days of propranolol treatment significantly lowered blood pressure in the older established spontaneous hypertensive rat and prevented the increases from occurring in the younger , developing hypertensive rat .
	manualset3
185577	6	414156	7	NULL	NULL	0	NULL	 occurring	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-five consecutive days of propranolol treatment significantly lowered blood pressure in the older established spontaneous hypertensive rat and prevented the increases from occurring in the younger , developing hypertensive rat .
	manualset3
183719	1	414157	7	NULL	NULL	0	NULL	Thirty-five homozygous deletions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-five homozygous deletions and 7 intragenic mutations of the pl6INK4/MTS1 gene were also detected in these cell lines .
	manualset3
183720	2	414157	7	NULL	NULL	0	NULL	7 intragenic mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-five homozygous deletions and 7 intragenic mutations of the pl6INK4/MTS1 gene were also detected in these cell lines .
	manualset3
183721	3	414157	7	NULL	NULL	0	NULL	pl6INK4/MTS1 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-five homozygous deletions and 7 intragenic mutations of the pl6INK4/MTS1 gene were also detected in these cell lines .
	manualset3
183722	4	414157	7	NULL	NULL	0	NULL	cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-five homozygous deletions and 7 intragenic mutations of the pl6INK4/MTS1 gene were also detected in these cell lines .
	manualset3
183723	1	414158	7	NULL	NULL	0	NULL	Thirty-five 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-five of 85 infants in the high-volume group acquired murmurs consistent with patent ductus arteriosus , and 11 of these 35 had congestive heart failure .
	manualset3
183724	2	414158	7	NULL	NULL	0	NULL	85 infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-five of 85 infants in the high-volume group acquired murmurs consistent with patent ductus arteriosus , and 11 of these 35 had congestive heart failure .
	manualset3
183725	3	414158	7	NULL	NULL	0	NULL	 high-volume group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-five of 85 infants in the high-volume group acquired murmurs consistent with patent ductus arteriosus , and 11 of these 35 had congestive heart failure .
	manualset3
183726	4	414158	7	NULL	NULL	0	NULL	murmurs 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-five of 85 infants in the high-volume group acquired murmurs consistent with patent ductus arteriosus , and 11 of these 35 had congestive heart failure .
	manualset3
183727	5	414158	7	NULL	NULL	0	NULL	patent ductus arteriosus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-five of 85 infants in the high-volume group acquired murmurs consistent with patent ductus arteriosus , and 11 of these 35 had congestive heart failure .
	manualset3
183728	6	414158	7	NULL	NULL	0	NULL	11	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-five of 85 infants in the high-volume group acquired murmurs consistent with patent ductus arteriosus , and 11 of these 35 had congestive heart failure .
	manualset3
183729	7	414158	7	NULL	NULL	0	NULL	35	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-five of 85 infants in the high-volume group acquired murmurs consistent with patent ductus arteriosus , and 11 of these 35 had congestive heart failure .
	manualset3
183730	8	414158	7	NULL	NULL	0	NULL	congestive heart failure 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-five of 85 infants in the high-volume group acquired murmurs consistent with patent ductus arteriosus , and 11 of these 35 had congestive heart failure .
	manualset3
183731	1	414159	7	NULL	NULL	0	NULL	Thirty-five patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-five patients who had angina at rest that was unresponsive to standard therapy comprised of oral or topical nitrates and beta-blocking drugs were treated with a continuous infusion of intravenous nitroglycerin ( IVNTG ) .
	manualset3
183732	2	414159	7	NULL	NULL	0	NULL	angina	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-five patients who had angina at rest that was unresponsive to standard therapy comprised of oral or topical nitrates and beta-blocking drugs were treated with a continuous infusion of intravenous nitroglycerin ( IVNTG ) .
	manualset3
183733	3	414159	7	NULL	NULL	0	NULL	rest	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-five patients who had angina at rest that was unresponsive to standard therapy comprised of oral or topical nitrates and beta-blocking drugs were treated with a continuous infusion of intravenous nitroglycerin ( IVNTG ) .
	manualset3
183734	4	414159	7	NULL	NULL	0	NULL	 standard therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-five patients who had angina at rest that was unresponsive to standard therapy comprised of oral or topical nitrates and beta-blocking drugs were treated with a continuous infusion of intravenous nitroglycerin ( IVNTG ) .
	manualset3
183735	5	414159	7	NULL	NULL	0	NULL	oral nitrates	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-five patients who had angina at rest that was unresponsive to standard therapy comprised of oral or topical nitrates and beta-blocking drugs were treated with a continuous infusion of intravenous nitroglycerin ( IVNTG ) .
	manualset3
183736	6	414159	7	NULL	NULL	0	NULL	topical nitrates	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-five patients who had angina at rest that was unresponsive to standard therapy comprised of oral or topical nitrates and beta-blocking drugs were treated with a continuous infusion of intravenous nitroglycerin ( IVNTG ) .
	manualset3
183737	7	414159	7	NULL	NULL	0	NULL	beta-blocking drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-five patients who had angina at rest that was unresponsive to standard therapy comprised of oral or topical nitrates and beta-blocking drugs were treated with a continuous infusion of intravenous nitroglycerin ( IVNTG ) .
	manualset3
183738	8	414159	7	NULL	NULL	0	NULL	continuous infusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-five patients who had angina at rest that was unresponsive to standard therapy comprised of oral or topical nitrates and beta-blocking drugs were treated with a continuous infusion of intravenous nitroglycerin ( IVNTG ) .
	manualset3
183739	9	414159	7	NULL	NULL	0	NULL	intravenous nitroglycerin ( IVNTG )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-five patients who had angina at rest that was unresponsive to standard therapy comprised of oral or topical nitrates and beta-blocking drugs were treated with a continuous infusion of intravenous nitroglycerin ( IVNTG ) .
	manualset3
183740	1	414160	7	NULL	NULL	0	NULL	Comparative study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative study of the influence of beta-adrenergic stimulants and adrenergic blocking drugs on renal function in normal humans ) .
	manualset3
183741	2	414160	7	NULL	NULL	0	NULL	beta-adrenergic stimulants	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative study of the influence of beta-adrenergic stimulants and adrenergic blocking drugs on renal function in normal humans ) .
	manualset3
183742	3	414160	7	NULL	NULL	0	NULL	adrenergic blocking drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative study of the influence of beta-adrenergic stimulants and adrenergic blocking drugs on renal function in normal humans ) .
	manualset3
183743	4	414160	7	NULL	NULL	0	NULL	renal function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative study of the influence of beta-adrenergic stimulants and adrenergic blocking drugs on renal function in normal humans ) .
	manualset3
183744	5	414160	7	NULL	NULL	0	NULL	normal humans 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparative study of the influence of beta-adrenergic stimulants and adrenergic blocking drugs on renal function in normal humans ) .
	manualset3
183745	1	414161	7	NULL	NULL	0	NULL	nanomaterial	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , this nanomaterial shows high performance in convenient magnetic separability and efficient removal of Hg ( 2 + ) .
	manualset3
183746	2	414161	7	NULL	NULL	0	NULL	high performance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , this nanomaterial shows high performance in convenient magnetic separability and efficient removal of Hg ( 2 + ) .
	manualset3
183747	3	414161	7	NULL	NULL	0	NULL	magnetic separability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , this nanomaterial shows high performance in convenient magnetic separability and efficient removal of Hg ( 2 + ) .
	manualset3
183748	4	414161	7	NULL	NULL	NULL	NULL	removal	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Additionally , this nanomaterial shows high performance in convenient magnetic separability and efficient removal of Hg ( 2 + ) .
	manualset3
185578	5	414161	7	NULL	NULL	0	NULL	Hg ( 2 + )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , this nanomaterial shows high performance in convenient magnetic separability and efficient removal of Hg ( 2 + ) .
	manualset3
183749	1	414162	7	NULL	NULL	0	NULL	Thirty-nine patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-nine patients with FHF ( 31 females , 8 males with mean age of 32.3 , range : 7-64 ) underwent TPE .
	manualset3
183750	2	414162	7	NULL	NULL	0	NULL	FHF	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-nine patients with FHF ( 31 females , 8 males with mean age of 32.3 , range : 7-64 ) underwent TPE .
	manualset3
183751	3	414162	7	NULL	NULL	0	NULL	31 females	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-nine patients with FHF ( 31 females , 8 males with mean age of 32.3 , range : 7-64 ) underwent TPE .
	manualset3
183752	4	414162	7	NULL	NULL	0	NULL	8 males	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-nine patients with FHF ( 31 females , 8 males with mean age of 32.3 , range : 7-64 ) underwent TPE .
	manualset3
183753	5	414162	7	NULL	NULL	0	NULL	mean age	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-nine patients with FHF ( 31 females , 8 males with mean age of 32.3 , range : 7-64 ) underwent TPE .
	manualset3
183754	6	414162	7	NULL	NULL	0	NULL	32.3	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-nine patients with FHF ( 31 females , 8 males with mean age of 32.3 , range : 7-64 ) underwent TPE .
	manualset3
183755	7	414162	7	NULL	NULL	0	NULL	range : 7-64	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-nine patients with FHF ( 31 females , 8 males with mean age of 32.3 , range : 7-64 ) underwent TPE .
	manualset3
183756	8	414162	7	NULL	NULL	0	NULL	TPE	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-nine patients with FHF ( 31 females , 8 males with mean age of 32.3 , range : 7-64 ) underwent TPE .
	manualset3
183757	1	414163	7	NULL	NULL	0	NULL	Thirty-nine viruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-nine viruses were 93.7 % to 94.3 % identical to FAdV07 strain x11a , but the genetic and immunogenic properties of this strain require further investigation .
	manualset3
183758	2	414163	7	NULL	NULL	0	NULL	93.7 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-nine viruses were 93.7 % to 94.3 % identical to FAdV07 strain x11a , but the genetic and immunogenic properties of this strain require further investigation .
	manualset3
183759	3	414163	7	NULL	NULL	0	NULL	94.3 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-nine viruses were 93.7 % to 94.3 % identical to FAdV07 strain x11a , but the genetic and immunogenic properties of this strain require further investigation .
	manualset3
183760	4	414163	7	NULL	NULL	0	NULL	FAdV07 strain x11a	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-nine viruses were 93.7 % to 94.3 % identical to FAdV07 strain x11a , but the genetic and immunogenic properties of this strain require further investigation .
	manualset3
183761	5	414163	7	NULL	NULL	0	NULL	genetic properties	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-nine viruses were 93.7 % to 94.3 % identical to FAdV07 strain x11a , but the genetic and immunogenic properties of this strain require further investigation .
	manualset3
183762	6	414163	7	NULL	NULL	0	NULL	 immunogenic properties	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-nine viruses were 93.7 % to 94.3 % identical to FAdV07 strain x11a , but the genetic and immunogenic properties of this strain require further investigation .
	manualset3
183763	7	414163	7	NULL	NULL	0	NULL	strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-nine viruses were 93.7 % to 94.3 % identical to FAdV07 strain x11a , but the genetic and immunogenic properties of this strain require further investigation .
	manualset3
183764	8	414163	7	NULL	NULL	0	NULL	investigation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-nine viruses were 93.7 % to 94.3 % identical to FAdV07 strain x11a , but the genetic and immunogenic properties of this strain require further investigation .
	manualset3
183765	1	414164	7	NULL	NULL	0	NULL	Thirty-six percent	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-six percent of the prisoners acknowledged using illicit drugs , primarily cocaine , during their pregnancies as compared to 3 % of the controls .
	manualset3
183766	2	414164	7	NULL	NULL	0	NULL	prisoners	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-six percent of the prisoners acknowledged using illicit drugs , primarily cocaine , during their pregnancies as compared to 3 % of the controls .
	manualset3
183767	3	414164	7	NULL	NULL	0	NULL	illicit drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-six percent of the prisoners acknowledged using illicit drugs , primarily cocaine , during their pregnancies as compared to 3 % of the controls .
	manualset3
183768	4	414164	7	NULL	NULL	0	NULL	cocaine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-six percent of the prisoners acknowledged using illicit drugs , primarily cocaine , during their pregnancies as compared to 3 % of the controls .
	manualset3
183769	5	414164	7	NULL	NULL	0	NULL	pregnancies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-six percent of the prisoners acknowledged using illicit drugs , primarily cocaine , during their pregnancies as compared to 3 % of the controls .
	manualset3
183770	6	414164	7	NULL	NULL	0	NULL	3 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-six percent of the prisoners acknowledged using illicit drugs , primarily cocaine , during their pregnancies as compared to 3 % of the controls .
	manualset3
183771	7	414164	7	NULL	NULL	0	NULL	controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-six percent of the prisoners acknowledged using illicit drugs , primarily cocaine , during their pregnancies as compared to 3 % of the controls .
	manualset3
183772	1	414165	7	NULL	NULL	0	NULL	Thirty-three cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-three cases were sufficiently documented to be considered as SSPE ( mean age on onset : 6.1 years ; male/female ratio : 3.7 ) .
	manualset3
183774	3	414165	7	NULL	NULL	0	NULL	SSPE	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-three cases were sufficiently documented to be considered as SSPE ( mean age on onset : 6.1 years ; male/female ratio : 3.7 ) .
	manualset3
183775	4	414165	7	NULL	NULL	0	NULL	mean age	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-three cases were sufficiently documented to be considered as SSPE ( mean age on onset : 6.1 years ; male/female ratio : 3.7 ) .
	manualset3
183776	5	414165	7	NULL	NULL	0	NULL	onset	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-three cases were sufficiently documented to be considered as SSPE ( mean age on onset : 6.1 years ; male/female ratio : 3.7 ) .
	manualset3
183777	6	414165	7	NULL	NULL	0	NULL	 6.1 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-three cases were sufficiently documented to be considered as SSPE ( mean age on onset : 6.1 years ; male/female ratio : 3.7 ) .
	manualset3
183778	7	414165	7	NULL	NULL	0	NULL	male/female ratio	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-three cases were sufficiently documented to be considered as SSPE ( mean age on onset : 6.1 years ; male/female ratio : 3.7 ) .
	manualset3
183779	8	414165	7	NULL	NULL	0	NULL	 3.7	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-three cases were sufficiently documented to be considered as SSPE ( mean age on onset : 6.1 years ; male/female ratio : 3.7 ) .
	manualset3
183780	1	414166	7	NULL	NULL	0	NULL	Thirty-three patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-three patients underwent total laryngectomy with primary pharyngeal closure , 14 patients had , in addition , pharyngectomy and pectoralis major myocutaneous flap reconstruction , and 5 patients had pharyngolaryngoesophagectomy and gastric transposition .
	manualset3
183781	2	414166	7	NULL	NULL	0	NULL	total laryngectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-three patients underwent total laryngectomy with primary pharyngeal closure , 14 patients had , in addition , pharyngectomy and pectoralis major myocutaneous flap reconstruction , and 5 patients had pharyngolaryngoesophagectomy and gastric transposition .
	manualset3
183782	3	414166	7	NULL	NULL	0	NULL	primary pharyngeal closure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-three patients underwent total laryngectomy with primary pharyngeal closure , 14 patients had , in addition , pharyngectomy and pectoralis major myocutaneous flap reconstruction , and 5 patients had pharyngolaryngoesophagectomy and gastric transposition .
	manualset3
183783	4	414166	7	NULL	NULL	0	NULL	14 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-three patients underwent total laryngectomy with primary pharyngeal closure , 14 patients had , in addition , pharyngectomy and pectoralis major myocutaneous flap reconstruction , and 5 patients had pharyngolaryngoesophagectomy and gastric transposition .
	manualset3
183784	5	414166	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-three patients underwent total laryngectomy with primary pharyngeal closure , 14 patients had , in addition , pharyngectomy and pectoralis major myocutaneous flap reconstruction , and 5 patients had pharyngolaryngoesophagectomy and gastric transposition .
	manualset3
183785	6	414166	7	NULL	NULL	0	NULL	pharyngectomy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-three patients underwent total laryngectomy with primary pharyngeal closure , 14 patients had , in addition , pharyngectomy and pectoralis major myocutaneous flap reconstruction , and 5 patients had pharyngolaryngoesophagectomy and gastric transposition .
	manualset3
183786	7	414166	7	NULL	NULL	0	NULL	pectoralis major myocutaneous flap reconstruction	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-three patients underwent total laryngectomy with primary pharyngeal closure , 14 patients had , in addition , pharyngectomy and pectoralis major myocutaneous flap reconstruction , and 5 patients had pharyngolaryngoesophagectomy and gastric transposition .
	manualset3
183787	8	414166	7	NULL	NULL	0	NULL	5 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-three patients underwent total laryngectomy with primary pharyngeal closure , 14 patients had , in addition , pharyngectomy and pectoralis major myocutaneous flap reconstruction , and 5 patients had pharyngolaryngoesophagectomy and gastric transposition .
	manualset3
183788	9	414166	7	NULL	NULL	0	NULL	pharyngolaryngoesophagectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-three patients underwent total laryngectomy with primary pharyngeal closure , 14 patients had , in addition , pharyngectomy and pectoralis major myocutaneous flap reconstruction , and 5 patients had pharyngolaryngoesophagectomy and gastric transposition .
	manualset3
183789	10	414166	7	NULL	NULL	0	NULL	gastric transposition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty-three patients underwent total laryngectomy with primary pharyngeal closure , 14 patients had , in addition , pharyngectomy and pectoralis major myocutaneous flap reconstruction , and 5 patients had pharyngolaryngoesophagectomy and gastric transposition .
	manualset3
183790	1	414167	7	NULL	NULL	0	NULL	underreporting	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , underreporting was associated with diets lower in fat ( P & lt ; 0.01 ) and alcohol ( P & lt ; 0.01 in women ) when expressed as a percentage of total energy intake .
	manualset3
183791	2	414167	7	NULL	NULL	0	NULL	 diets	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , underreporting was associated with diets lower in fat ( P & lt ; 0.01 ) and alcohol ( P & lt ; 0.01 in women ) when expressed as a percentage of total energy intake .
	manualset3
183792	3	414167	7	NULL	NULL	0	NULL	fat 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , underreporting was associated with diets lower in fat ( P & lt ; 0.01 ) and alcohol ( P & lt ; 0.01 in women ) when expressed as a percentage of total energy intake .
	manualset3
183793	4	414167	7	NULL	NULL	0	NULL	P & lt ; 0.01 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , underreporting was associated with diets lower in fat ( P & lt ; 0.01 ) and alcohol ( P & lt ; 0.01 in women ) when expressed as a percentage of total energy intake .
	manualset3
183794	5	414167	7	NULL	NULL	0	NULL	alcohol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , underreporting was associated with diets lower in fat ( P & lt ; 0.01 ) and alcohol ( P & lt ; 0.01 in women ) when expressed as a percentage of total energy intake .
	manualset3
183795	6	414167	7	NULL	NULL	0	NULL	P & lt ; 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , underreporting was associated with diets lower in fat ( P & lt ; 0.01 ) and alcohol ( P & lt ; 0.01 in women ) when expressed as a percentage of total energy intake .
	manualset3
183796	7	414167	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , underreporting was associated with diets lower in fat ( P & lt ; 0.01 ) and alcohol ( P & lt ; 0.01 in women ) when expressed as a percentage of total energy intake .
	manualset3
183797	8	414167	7	NULL	NULL	0	NULL	 percentage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , underreporting was associated with diets lower in fat ( P & lt ; 0.01 ) and alcohol ( P & lt ; 0.01 in women ) when expressed as a percentage of total energy intake .
	manualset3
183798	9	414167	7	NULL	NULL	0	NULL	total energy intake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , underreporting was associated with diets lower in fat ( P & lt ; 0.01 ) and alcohol ( P & lt ; 0.01 in women ) when expressed as a percentage of total energy intake .
	manualset3
183799	1	414168	7	NULL	NULL	NULL	NULL	Thirty hospitalized burn patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Thirty hospitalized burn patients and their nurses submitted visual analog scales ( VAS ) for pain during 2 consecutive daily wound debridements .
	manualset3
183800	2	414168	7	NULL	NULL	0	NULL	 nurses	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty hospitalized burn patients and their nurses submitted visual analog scales ( VAS ) for pain during 2 consecutive daily wound debridements .
	manualset3
183801	3	414168	7	NULL	NULL	0	NULL	visual analog scales ( VAS )	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty hospitalized burn patients and their nurses submitted visual analog scales ( VAS ) for pain during 2 consecutive daily wound debridements .
	manualset3
183802	4	414168	7	NULL	NULL	0	NULL	pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty hospitalized burn patients and their nurses submitted visual analog scales ( VAS ) for pain during 2 consecutive daily wound debridements .
	manualset3
183803	5	414168	7	NULL	NULL	0	NULL	2 consecutive daily wound debridements	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty hospitalized burn patients and their nurses submitted visual analog scales ( VAS ) for pain during 2 consecutive daily wound debridements .
	manualset3
183804	1	414169	7	NULL	NULL	NULL	NULL	Thirty patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Thirty patients diagnosed as suffering from endogenous depression were entered into a 3-week double-blind trial comparing three times a day dosage of dothiepin with a single night-time dosage in a dosage range of 75 mg to 225 mg per day .
	manualset3
183805	2	414169	7	NULL	NULL	0	NULL	endogenous depression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty patients diagnosed as suffering from endogenous depression were entered into a 3-week double-blind trial comparing three times a day dosage of dothiepin with a single night-time dosage in a dosage range of 75 mg to 225 mg per day .
	manualset3
183806	3	414169	7	NULL	NULL	0	NULL	3-week double-blind trial	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty patients diagnosed as suffering from endogenous depression were entered into a 3-week double-blind trial comparing three times a day dosage of dothiepin with a single night-time dosage in a dosage range of 75 mg to 225 mg per day .
	manualset3
183807	4	414169	7	NULL	NULL	0	NULL	three times	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty patients diagnosed as suffering from endogenous depression were entered into a 3-week double-blind trial comparing three times a day dosage of dothiepin with a single night-time dosage in a dosage range of 75 mg to 225 mg per day .
	manualset3
183808	5	414169	7	NULL	NULL	NULL	NULL	day dosage	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Thirty patients diagnosed as suffering from endogenous depression were entered into a 3-week double-blind trial comparing three times a day dosage of dothiepin with a single night-time dosage in a dosage range of 75 mg to 225 mg per day .
	manualset3
183809	6	414169	7	NULL	NULL	0	NULL	dothiepin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty patients diagnosed as suffering from endogenous depression were entered into a 3-week double-blind trial comparing three times a day dosage of dothiepin with a single night-time dosage in a dosage range of 75 mg to 225 mg per day .
	manualset3
183810	7	414169	7	NULL	NULL	NULL	NULL	single night-time dosage	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Thirty patients diagnosed as suffering from endogenous depression were entered into a 3-week double-blind trial comparing three times a day dosage of dothiepin with a single night-time dosage in a dosage range of 75 mg to 225 mg per day .
	manualset3
183811	8	414169	7	NULL	NULL	0	NULL	dosage range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty patients diagnosed as suffering from endogenous depression were entered into a 3-week double-blind trial comparing three times a day dosage of dothiepin with a single night-time dosage in a dosage range of 75 mg to 225 mg per day .
	manualset3
183812	9	414169	7	NULL	NULL	NULL	NULL	75 mg per day	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Thirty patients diagnosed as suffering from endogenous depression were entered into a 3-week double-blind trial comparing three times a day dosage of dothiepin with a single night-time dosage in a dosage range of 75 mg to 225 mg per day .
	manualset3
183813	10	414169	7	NULL	NULL	0	NULL	225 mg per day	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty patients diagnosed as suffering from endogenous depression were entered into a 3-week double-blind trial comparing three times a day dosage of dothiepin with a single night-time dosage in a dosage range of 75 mg to 225 mg per day .
	manualset3
183814	1	414170	7	NULL	NULL	0	NULL	Thirty tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty tumors ( 93.8 % ) expressed vimentin , 15 ( 46.9 % ) marked for alpha 1AChy , 11 ( 34.4 % ) exhibited alpha 1AT , and 11 ( 34.4 % ) expressed S-100 protein .
	manualset3
183815	2	414170	7	NULL	NULL	0	NULL	 93.8 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty tumors ( 93.8 % ) expressed vimentin , 15 ( 46.9 % ) marked for alpha 1AChy , 11 ( 34.4 % ) exhibited alpha 1AT , and 11 ( 34.4 % ) expressed S-100 protein .
	manualset3
183816	3	414170	7	NULL	NULL	0	NULL	vimentin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty tumors ( 93.8 % ) expressed vimentin , 15 ( 46.9 % ) marked for alpha 1AChy , 11 ( 34.4 % ) exhibited alpha 1AT , and 11 ( 34.4 % ) expressed S-100 protein .
	manualset3
183817	4	414170	7	NULL	NULL	0	NULL	15 ( 46.9 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty tumors ( 93.8 % ) expressed vimentin , 15 ( 46.9 % ) marked for alpha 1AChy , 11 ( 34.4 % ) exhibited alpha 1AT , and 11 ( 34.4 % ) expressed S-100 protein .
	manualset3
183818	5	414170	7	NULL	NULL	0	NULL	alpha 1AChy 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty tumors ( 93.8 % ) expressed vimentin , 15 ( 46.9 % ) marked for alpha 1AChy , 11 ( 34.4 % ) exhibited alpha 1AT , and 11 ( 34.4 % ) expressed S-100 protein .
	manualset3
183819	6	414170	7	NULL	NULL	0	NULL	11 ( 34.4 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty tumors ( 93.8 % ) expressed vimentin , 15 ( 46.9 % ) marked for alpha 1AChy , 11 ( 34.4 % ) exhibited alpha 1AT , and 11 ( 34.4 % ) expressed S-100 protein .
	manualset3
183820	7	414170	7	NULL	NULL	0	NULL	alpha 1AT	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty tumors ( 93.8 % ) expressed vimentin , 15 ( 46.9 % ) marked for alpha 1AChy , 11 ( 34.4 % ) exhibited alpha 1AT , and 11 ( 34.4 % ) expressed S-100 protein .
	manualset3
183821	8	414170	7	NULL	NULL	0	NULL	11 ( 34.4 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty tumors ( 93.8 % ) expressed vimentin , 15 ( 46.9 % ) marked for alpha 1AChy , 11 ( 34.4 % ) exhibited alpha 1AT , and 11 ( 34.4 % ) expressed S-100 protein .
	manualset3
183822	9	414170	7	NULL	NULL	0	NULL	S-100 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty tumors ( 93.8 % ) expressed vimentin , 15 ( 46.9 % ) marked for alpha 1AChy , 11 ( 34.4 % ) exhibited alpha 1AT , and 11 ( 34.4 % ) expressed S-100 protein .
	manualset3
183823	1	414171	7	NULL	NULL	0	NULL	high reproductive potential	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This , along with the utility and high reproductive potential of fish species such as Danio rerio , Oryzias latipes etc. , suggests that fishes may provide ideal comparative biological models to facilitate a better understanding of this poorly understood region of the heart .
	manualset3
183824	2	414171	7	NULL	NULL	0	NULL	fish species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	This , along with the utility and high reproductive potential of fish species such as Danio rerio , Oryzias latipes etc. , suggests that fishes may provide ideal comparative biological models to facilitate a better understanding of this poorly understood region of the heart .
	manualset3
183825	3	414171	7	NULL	NULL	0	NULL	Danio rerio	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	This , along with the utility and high reproductive potential of fish species such as Danio rerio , Oryzias latipes etc. , suggests that fishes may provide ideal comparative biological models to facilitate a better understanding of this poorly understood region of the heart .
	manualset3
183826	4	414171	7	NULL	NULL	0	NULL	Oryzias latipes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	This , along with the utility and high reproductive potential of fish species such as Danio rerio , Oryzias latipes etc. , suggests that fishes may provide ideal comparative biological models to facilitate a better understanding of this poorly understood region of the heart .
	manualset3
183827	5	414171	7	NULL	NULL	0	NULL	fishes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	This , along with the utility and high reproductive potential of fish species such as Danio rerio , Oryzias latipes etc. , suggests that fishes may provide ideal comparative biological models to facilitate a better understanding of this poorly understood region of the heart .
	manualset3
183828	6	414171	7	NULL	NULL	0	NULL	comparative biological models	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	This , along with the utility and high reproductive potential of fish species such as Danio rerio , Oryzias latipes etc. , suggests that fishes may provide ideal comparative biological models to facilitate a better understanding of this poorly understood region of the heart .
	manualset3
183829	7	414171	7	NULL	NULL	0	NULL	understanding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This , along with the utility and high reproductive potential of fish species such as Danio rerio , Oryzias latipes etc. , suggests that fishes may provide ideal comparative biological models to facilitate a better understanding of this poorly understood region of the heart .
	manualset3
183830	8	414171	7	NULL	NULL	0	NULL	region of the heart 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This , along with the utility and high reproductive potential of fish species such as Danio rerio , Oryzias latipes etc. , suggests that fishes may provide ideal comparative biological models to facilitate a better understanding of this poorly understood region of the heart .
	manualset3
183831	1	414172	7	NULL	NULL	0	NULL	questions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This , in turn , raises questions about the timing of organogenesis and gestational comparability in cebid and cercopithecid monkeys .
	manualset3
183832	2	414172	7	NULL	NULL	0	NULL	timing	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	This , in turn , raises questions about the timing of organogenesis and gestational comparability in cebid and cercopithecid monkeys .
	manualset3
183833	3	414172	7	NULL	NULL	0	NULL	organogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This , in turn , raises questions about the timing of organogenesis and gestational comparability in cebid and cercopithecid monkeys .
	manualset3
183834	4	414172	7	NULL	NULL	0	NULL	gestational comparability 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This , in turn , raises questions about the timing of organogenesis and gestational comparability in cebid and cercopithecid monkeys .
	manualset3
183835	5	414172	7	NULL	NULL	0	NULL	cebid monkeys	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	This , in turn , raises questions about the timing of organogenesis and gestational comparability in cebid and cercopithecid monkeys .
	manualset3
183836	6	414172	7	NULL	NULL	0	NULL	cercopithecid monkeys	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	This , in turn , raises questions about the timing of organogenesis and gestational comparability in cebid and cercopithecid monkeys .
	manualset3
183838	1	414173	7	NULL	NULL	0	NULL	bone marrow-derived cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , we show that bone marrow-derived cells can be identified in the liver without prior sex-mismatch bone marrow transplantation , identifying instead the BCR : ABL fusion gene that is present in all such cells in almost all patients suffering from chronic myelogenous leukemia ( CML ) .
	manualset3
183839	2	414173	7	NULL	NULL	0	NULL	 liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , we show that bone marrow-derived cells can be identified in the liver without prior sex-mismatch bone marrow transplantation , identifying instead the BCR : ABL fusion gene that is present in all such cells in almost all patients suffering from chronic myelogenous leukemia ( CML ) .
	manualset3
183840	3	414173	7	NULL	NULL	0	NULL	sex-mismatch bone marrow transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , we show that bone marrow-derived cells can be identified in the liver without prior sex-mismatch bone marrow transplantation , identifying instead the BCR : ABL fusion gene that is present in all such cells in almost all patients suffering from chronic myelogenous leukemia ( CML ) .
	manualset3
183841	4	414173	7	NULL	NULL	0	NULL	BCR : ABL fusion gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , we show that bone marrow-derived cells can be identified in the liver without prior sex-mismatch bone marrow transplantation , identifying instead the BCR : ABL fusion gene that is present in all such cells in almost all patients suffering from chronic myelogenous leukemia ( CML ) .
	manualset3
183842	5	414173	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , we show that bone marrow-derived cells can be identified in the liver without prior sex-mismatch bone marrow transplantation , identifying instead the BCR : ABL fusion gene that is present in all such cells in almost all patients suffering from chronic myelogenous leukemia ( CML ) .
	manualset3
183843	6	414173	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , we show that bone marrow-derived cells can be identified in the liver without prior sex-mismatch bone marrow transplantation , identifying instead the BCR : ABL fusion gene that is present in all such cells in almost all patients suffering from chronic myelogenous leukemia ( CML ) .
	manualset3
183844	7	414173	7	NULL	NULL	0	NULL	chronic myelogenous leukemia ( CML )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , we show that bone marrow-derived cells can be identified in the liver without prior sex-mismatch bone marrow transplantation , identifying instead the BCR : ABL fusion gene that is present in all such cells in almost all patients suffering from chronic myelogenous leukemia ( CML ) .
	manualset3
183845	1	414174	7	NULL	NULL	0	NULL	Missouri Medicine series 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	This , the second in a Missouri Medicine series on stroke , summarizes the available acute treatment options and the evolving role of neuro-imaging in directing therapeutic decisions .
	manualset3
183846	2	414174	7	NULL	NULL	0	NULL	 stroke	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This , the second in a Missouri Medicine series on stroke , summarizes the available acute treatment options and the evolving role of neuro-imaging in directing therapeutic decisions .
	manualset3
183847	3	414174	7	NULL	NULL	0	NULL	acute treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This , the second in a Missouri Medicine series on stroke , summarizes the available acute treatment options and the evolving role of neuro-imaging in directing therapeutic decisions .
	manualset3
183848	4	414174	7	NULL	NULL	0	NULL	evolving role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This , the second in a Missouri Medicine series on stroke , summarizes the available acute treatment options and the evolving role of neuro-imaging in directing therapeutic decisions .
	manualset3
183849	5	414174	7	NULL	NULL	0	NULL	neuro-imaging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This , the second in a Missouri Medicine series on stroke , summarizes the available acute treatment options and the evolving role of neuro-imaging in directing therapeutic decisions .
	manualset3
183850	6	414174	7	NULL	NULL	0	NULL	therapeutic decisions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This , the second in a Missouri Medicine series on stroke , summarizes the available acute treatment options and the evolving role of neuro-imaging in directing therapeutic decisions .
	manualset3
183851	1	414175	7	NULL	NULL	0	NULL	 anatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This , together with the presence of anatase , a low-temperature polymorph of TiO ( 2 ) , suggested that some regions of the fulgurite specimen were not subjected to temperatures of 1800 degrees C , which are attained when lightning hits the surface of sand or a rock .
	manualset3
183852	2	414175	7	NULL	NULL	0	NULL	low-temperature polymorph	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This , together with the presence of anatase , a low-temperature polymorph of TiO ( 2 ) , suggested that some regions of the fulgurite specimen were not subjected to temperatures of 1800 degrees C , which are attained when lightning hits the surface of sand or a rock .
	manualset3
183853	3	414175	7	NULL	NULL	0	NULL	TiO ( 2 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This , together with the presence of anatase , a low-temperature polymorph of TiO ( 2 ) , suggested that some regions of the fulgurite specimen were not subjected to temperatures of 1800 degrees C , which are attained when lightning hits the surface of sand or a rock .
	manualset3
183854	4	414175	7	NULL	NULL	0	NULL	 regions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This , together with the presence of anatase , a low-temperature polymorph of TiO ( 2 ) , suggested that some regions of the fulgurite specimen were not subjected to temperatures of 1800 degrees C , which are attained when lightning hits the surface of sand or a rock .
	manualset3
183855	5	414175	7	NULL	NULL	0	NULL	fulgurite specimen	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This , together with the presence of anatase , a low-temperature polymorph of TiO ( 2 ) , suggested that some regions of the fulgurite specimen were not subjected to temperatures of 1800 degrees C , which are attained when lightning hits the surface of sand or a rock .
	manualset3
183856	6	414175	7	NULL	NULL	0	NULL	 temperatures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This , together with the presence of anatase , a low-temperature polymorph of TiO ( 2 ) , suggested that some regions of the fulgurite specimen were not subjected to temperatures of 1800 degrees C , which are attained when lightning hits the surface of sand or a rock .
	manualset3
183857	7	414175	7	NULL	NULL	0	NULL	1800 degrees C	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This , together with the presence of anatase , a low-temperature polymorph of TiO ( 2 ) , suggested that some regions of the fulgurite specimen were not subjected to temperatures of 1800 degrees C , which are attained when lightning hits the surface of sand or a rock .
	manualset3
183858	8	414175	7	NULL	NULL	0	NULL	lightning 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This , together with the presence of anatase , a low-temperature polymorph of TiO ( 2 ) , suggested that some regions of the fulgurite specimen were not subjected to temperatures of 1800 degrees C , which are attained when lightning hits the surface of sand or a rock .
	manualset3
183859	9	414175	7	NULL	NULL	0	NULL	surface of sand 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	This , together with the presence of anatase , a low-temperature polymorph of TiO ( 2 ) , suggested that some regions of the fulgurite specimen were not subjected to temperatures of 1800 degrees C , which are attained when lightning hits the surface of sand or a rock .
	manualset3
183860	10	414175	7	NULL	NULL	0	NULL	 rock	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	This , together with the presence of anatase , a low-temperature polymorph of TiO ( 2 ) , suggested that some regions of the fulgurite specimen were not subjected to temperatures of 1800 degrees C , which are attained when lightning hits the surface of sand or a rock .
	manualset3
183861	1	414176	7	NULL	NULL	NULL	NULL	EOM sample	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This EOM sample induced a nearly two-fold lower level of DNA damage in comparison with other EOMs .
	manualset3
183862	2	414176	7	NULL	NULL	0	NULL	lower level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This EOM sample induced a nearly two-fold lower level of DNA damage in comparison with other EOMs .
	manualset3
183863	3	414176	7	NULL	NULL	0	NULL	DNA damage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This EOM sample induced a nearly two-fold lower level of DNA damage in comparison with other EOMs .
	manualset3
183864	4	414176	7	NULL	NULL	0	NULL	comparison 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	This EOM sample induced a nearly two-fold lower level of DNA damage in comparison with other EOMs .
	manualset3
183865	5	414176	7	NULL	NULL	0	NULL	EOMs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This EOM sample induced a nearly two-fold lower level of DNA damage in comparison with other EOMs .
	manualset3
183866	1	414177	7	NULL	NULL	0	NULL	KTC-2 cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	This KTC-2 cell line may be a suitable model for developing new strategies against paraneoplastic syndromes caused by anaplastic thyroid cancer .
	manualset3
183867	2	414177	7	NULL	NULL	0	NULL	 model 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	This KTC-2 cell line may be a suitable model for developing new strategies against paraneoplastic syndromes caused by anaplastic thyroid cancer .
	manualset3
183868	3	414177	7	NULL	NULL	0	NULL	new strategies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This KTC-2 cell line may be a suitable model for developing new strategies against paraneoplastic syndromes caused by anaplastic thyroid cancer .
	manualset3
183869	4	414177	7	NULL	NULL	0	NULL	paraneoplastic syndromes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This KTC-2 cell line may be a suitable model for developing new strategies against paraneoplastic syndromes caused by anaplastic thyroid cancer .
	manualset3
183870	5	414177	7	NULL	NULL	0	NULL	anaplastic thyroid cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This KTC-2 cell line may be a suitable model for developing new strategies against paraneoplastic syndromes caused by anaplastic thyroid cancer .
	manualset3
185580	6	414177	7	NULL	NULL	0	NULL	developing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This KTC-2 cell line may be a suitable model for developing new strategies against paraneoplastic syndromes caused by anaplastic thyroid cancer .
	manualset3
183871	1	414178	7	NULL	NULL	0	NULL	L-DOPA release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This L-DOPA release was suppressed by acute lesion in the ipsilateral nucleus tractus solitarii .
	manualset3
183872	2	414178	7	NULL	NULL	0	NULL	acute lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This L-DOPA release was suppressed by acute lesion in the ipsilateral nucleus tractus solitarii .
	manualset3
183873	3	414178	7	NULL	NULL	0	NULL	 ipsilateral nucleus tractus solitarii 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	This L-DOPA release was suppressed by acute lesion in the ipsilateral nucleus tractus solitarii .
	manualset3
183874	1	414179	7	NULL	NULL	0	NULL	RAS	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This RAS appears to differ from the circulating and the local RAS , in terms of components and the mechanism of action .
	manualset3
183875	2	414179	7	NULL	NULL	0	NULL	 circulating RAS	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This RAS appears to differ from the circulating and the local RAS , in terms of components and the mechanism of action .
	manualset3
183876	3	414179	7	NULL	NULL	0	NULL	local RAS	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This RAS appears to differ from the circulating and the local RAS , in terms of components and the mechanism of action .
	manualset3
183877	4	414179	7	NULL	NULL	NULL	NULL	components	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This RAS appears to differ from the circulating and the local RAS , in terms of components and the mechanism of action .
	manualset3
183878	5	414179	7	NULL	NULL	0	NULL	mechanism of action	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This RAS appears to differ from the circulating and the local RAS , in terms of components and the mechanism of action .
	manualset3
183879	1	414180	7	NULL	NULL	0	NULL	SNP	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	This SNP maps to an intronic region of the SPATA5 ( spermatogenesis-associated protein 5 ) gene on chromosome 4 .
	manualset3
183880	2	414180	7	NULL	NULL	0	NULL	intronic region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	This SNP maps to an intronic region of the SPATA5 ( spermatogenesis-associated protein 5 ) gene on chromosome 4 .
	manualset3
183881	3	414180	7	NULL	NULL	0	NULL	SPATA5 ( spermatogenesis-associated protein 5 ) gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	This SNP maps to an intronic region of the SPATA5 ( spermatogenesis-associated protein 5 ) gene on chromosome 4 .
	manualset3
183882	4	414180	7	NULL	NULL	0	NULL	chromosome 4	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	This SNP maps to an intronic region of the SPATA5 ( spermatogenesis-associated protein 5 ) gene on chromosome 4 .
	manualset3
183883	1	414181	7	NULL	NULL	0	NULL	 dilute acid hydrolysis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally dilute acid hydrolysis of PTH , labeled with ( 35S ) methionine and containing 32P , generated an 35S-labeled fragment with which 32P co-chromatographed .
	manualset3
183884	2	414181	7	NULL	NULL	0	NULL	PTH	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally dilute acid hydrolysis of PTH , labeled with ( 35S ) methionine and containing 32P , generated an 35S-labeled fragment with which 32P co-chromatographed .
	manualset3
183885	3	414181	7	NULL	NULL	0	NULL	( 35S ) methionine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally dilute acid hydrolysis of PTH , labeled with ( 35S ) methionine and containing 32P , generated an 35S-labeled fragment with which 32P co-chromatographed .
	manualset3
183886	4	414181	7	NULL	NULL	0	NULL	32P	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally dilute acid hydrolysis of PTH , labeled with ( 35S ) methionine and containing 32P , generated an 35S-labeled fragment with which 32P co-chromatographed .
	manualset3
183887	5	414181	7	NULL	NULL	0	NULL	35S-labeled fragment	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally dilute acid hydrolysis of PTH , labeled with ( 35S ) methionine and containing 32P , generated an 35S-labeled fragment with which 32P co-chromatographed .
	manualset3
183888	6	414181	7	NULL	NULL	0	NULL	32P	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally dilute acid hydrolysis of PTH , labeled with ( 35S ) methionine and containing 32P , generated an 35S-labeled fragment with which 32P co-chromatographed .
	manualset3
183889	1	414182	7	NULL	NULL	0	NULL	ability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This ability of decreased NA activity to promote H5N1 infection underlines the necessity to optimize management strategies for a plausible H5N1 pandemic .
	manualset3
183890	2	414182	7	NULL	NULL	0	NULL	NA activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This ability of decreased NA activity to promote H5N1 infection underlines the necessity to optimize management strategies for a plausible H5N1 pandemic .
	manualset3
183891	3	414182	7	NULL	NULL	0	NULL	H5N1 infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This ability of decreased NA activity to promote H5N1 infection underlines the necessity to optimize management strategies for a plausible H5N1 pandemic .
	manualset3
183892	4	414182	7	NULL	NULL	0	NULL	management strategies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This ability of decreased NA activity to promote H5N1 infection underlines the necessity to optimize management strategies for a plausible H5N1 pandemic .
	manualset3
183893	5	414182	7	NULL	NULL	0	NULL	H5N1 pandemic	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This ability of decreased NA activity to promote H5N1 infection underlines the necessity to optimize management strategies for a plausible H5N1 pandemic .
	manualset3
183894	1	414183	7	NULL	NULL	0	NULL	absence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This absence of a response is interpreted as an adaptational deficit in reaction to variations in atmospheric parameters .
	manualset3
183895	2	414183	7	NULL	NULL	NULL	NULL	 response	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This absence of a response is interpreted as an adaptational deficit in reaction to variations in atmospheric parameters .
	manualset3
183896	3	414183	7	NULL	NULL	0	NULL	 adaptational deficit	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This absence of a response is interpreted as an adaptational deficit in reaction to variations in atmospheric parameters .
	manualset3
183897	4	414183	7	NULL	NULL	NULL	NULL	reaction 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This absence of a response is interpreted as an adaptational deficit in reaction to variations in atmospheric parameters .
	manualset3
183898	5	414183	7	NULL	NULL	NULL	NULL	variations	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This absence of a response is interpreted as an adaptational deficit in reaction to variations in atmospheric parameters .
	manualset3
183899	6	414183	7	NULL	NULL	0	NULL	atmospheric parameters	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	This absence of a response is interpreted as an adaptational deficit in reaction to variations in atmospheric parameters .
	manualset3
183900	1	414184	7	NULL	NULL	0	NULL	absence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This absence of negative regulatory activity occurred whether transfections were performed in human , rat or mouse hepatoma cell lines .
	manualset3
183901	2	414184	7	NULL	NULL	0	NULL	negative regulatory activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This absence of negative regulatory activity occurred whether transfections were performed in human , rat or mouse hepatoma cell lines .
	manualset3
183902	3	414184	7	NULL	NULL	0	NULL	 transfections	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This absence of negative regulatory activity occurred whether transfections were performed in human , rat or mouse hepatoma cell lines .
	manualset3
183903	4	414184	7	NULL	NULL	0	NULL	 human hepatoma cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	This absence of negative regulatory activity occurred whether transfections were performed in human , rat or mouse hepatoma cell lines .
	manualset3
183904	5	414184	7	NULL	NULL	0	NULL	rat hepatoma cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	This absence of negative regulatory activity occurred whether transfections were performed in human , rat or mouse hepatoma cell lines .
	manualset3
183905	6	414184	7	NULL	NULL	0	NULL	mouse hepatoma cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	This absence of negative regulatory activity occurred whether transfections were performed in human , rat or mouse hepatoma cell lines .
	manualset3
183906	1	414185	7	NULL	NULL	0	NULL	account 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This account reports direct evidence for the validation of the model through FT-IR spectroscopy and through a new method for `` titrating '' the binding sites via EPR spectroscopy .
	manualset3
183907	2	414185	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This account reports direct evidence for the validation of the model through FT-IR spectroscopy and through a new method for `` titrating '' the binding sites via EPR spectroscopy .
	manualset3
183908	3	414185	7	NULL	NULL	0	NULL	validation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This account reports direct evidence for the validation of the model through FT-IR spectroscopy and through a new method for `` titrating '' the binding sites via EPR spectroscopy .
	manualset3
183909	4	414185	7	NULL	NULL	0	NULL	model 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	This account reports direct evidence for the validation of the model through FT-IR spectroscopy and through a new method for `` titrating '' the binding sites via EPR spectroscopy .
	manualset3
183910	5	414185	7	NULL	NULL	0	NULL	FT-IR spectroscopy 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This account reports direct evidence for the validation of the model through FT-IR spectroscopy and through a new method for `` titrating '' the binding sites via EPR spectroscopy .
	manualset3
183911	6	414185	7	NULL	NULL	0	NULL	new method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This account reports direct evidence for the validation of the model through FT-IR spectroscopy and through a new method for `` titrating '' the binding sites via EPR spectroscopy .
	manualset3
183912	7	414185	7	NULL	NULL	NULL	NULL	`` titrating '' 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This account reports direct evidence for the validation of the model through FT-IR spectroscopy and through a new method for `` titrating '' the binding sites via EPR spectroscopy .
	manualset3
183913	8	414185	7	NULL	NULL	0	NULL	EPR spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This account reports direct evidence for the validation of the model through FT-IR spectroscopy and through a new method for `` titrating '' the binding sites via EPR spectroscopy .
	manualset3
185581	9	414185	7	NULL	NULL	0	NULL	 binding sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	This account reports direct evidence for the validation of the model through FT-IR spectroscopy and through a new method for `` titrating '' the binding sites via EPR spectroscopy .
	manualset3
183914	1	414186	7	NULL	NULL	0	NULL	activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This activity delayed the incidence of virus-induced diabetes and improved survival rates .
	manualset3
183915	2	414186	7	NULL	NULL	0	NULL	incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This activity delayed the incidence of virus-induced diabetes and improved survival rates .
	manualset3
183916	3	414186	7	NULL	NULL	0	NULL	virus-induced diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This activity delayed the incidence of virus-induced diabetes and improved survival rates .
	manualset3
183917	4	414186	7	NULL	NULL	0	NULL	survival rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This activity delayed the incidence of virus-induced diabetes and improved survival rates .
	manualset3
183918	1	414187	7	NULL	NULL	0	NULL	 correlation analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally performed the correlation analysis between pI ( calc ) and pI ( exp ) values for identified peptides proved the possibility to obtain experimentally useful high correlation .
	manualset3
183919	2	414187	7	NULL	NULL	0	NULL	pI ( calc ) values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally performed the correlation analysis between pI ( calc ) and pI ( exp ) values for identified peptides proved the possibility to obtain experimentally useful high correlation .
	manualset3
183920	3	414187	7	NULL	NULL	0	NULL	pI ( exp ) values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally performed the correlation analysis between pI ( calc ) and pI ( exp ) values for identified peptides proved the possibility to obtain experimentally useful high correlation .
	manualset3
183921	4	414187	7	NULL	NULL	0	NULL	peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally performed the correlation analysis between pI ( calc ) and pI ( exp ) values for identified peptides proved the possibility to obtain experimentally useful high correlation .
	manualset3
183922	5	414187	7	NULL	NULL	0	NULL	high correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally performed the correlation analysis between pI ( calc ) and pI ( exp ) values for identified peptides proved the possibility to obtain experimentally useful high correlation .
	manualset3
185582	6	414187	7	NULL	NULL	0	NULL	possibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally performed the correlation analysis between pI ( calc ) and pI ( exp ) values for identified peptides proved the possibility to obtain experimentally useful high correlation .
	manualset3
183923	1	414188	7	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This activity is believed to be largely due to the ability of the drug to inhibit the synthesis of prostaglandins .
	manualset3
183924	2	414188	7	NULL	NULL	0	NULL	ability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This activity is believed to be largely due to the ability of the drug to inhibit the synthesis of prostaglandins .
	manualset3
183925	3	414188	7	NULL	NULL	0	NULL	 drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	This activity is believed to be largely due to the ability of the drug to inhibit the synthesis of prostaglandins .
	manualset3
183926	4	414188	7	NULL	NULL	0	NULL	synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This activity is believed to be largely due to the ability of the drug to inhibit the synthesis of prostaglandins .
	manualset3
183927	5	414188	7	NULL	NULL	0	NULL	prostaglandins	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This activity is believed to be largely due to the ability of the drug to inhibit the synthesis of prostaglandins .
	manualset3
183928	1	414189	7	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This alternative role for PKR prevents penetration of virions into the cell .
	manualset3
183929	2	414189	7	NULL	NULL	0	NULL	PKR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This alternative role for PKR prevents penetration of virions into the cell .
	manualset3
183930	3	414189	7	NULL	NULL	0	NULL	 penetration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This alternative role for PKR prevents penetration of virions into the cell .
	manualset3
183931	4	414189	7	NULL	NULL	0	NULL	virions 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This alternative role for PKR prevents penetration of virions into the cell .
	manualset3
183932	5	414189	7	NULL	NULL	0	NULL	cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	This alternative role for PKR prevents penetration of virions into the cell .
	manualset3
183933	1	414190	7	NULL	NULL	0	NULL	amnesia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This amnesia for extinction disappeared with longer postextinction delays , demonstrating a temporal gradient .
	manualset3
183934	2	414190	7	NULL	NULL	0	NULL	extinction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This amnesia for extinction disappeared with longer postextinction delays , demonstrating a temporal gradient .
	manualset3
183935	3	414190	7	NULL	NULL	0	NULL	longer postextinction delays	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This amnesia for extinction disappeared with longer postextinction delays , demonstrating a temporal gradient .
	manualset3
183936	4	414190	7	NULL	NULL	0	NULL	temporal gradient	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This amnesia for extinction disappeared with longer postextinction delays , demonstrating a temporal gradient .
	manualset3
183937	1	414191	7	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This analysis examines the affect of 2 healthcare strategies on the rate of avoidable hospitalization , managed care and the healthcare safety net .
	manualset3
183938	2	414191	7	NULL	NULL	0	NULL	2 healthcare strategies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This analysis examines the affect of 2 healthcare strategies on the rate of avoidable hospitalization , managed care and the healthcare safety net .
	manualset3
183939	3	414191	7	NULL	NULL	0	NULL	rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This analysis examines the affect of 2 healthcare strategies on the rate of avoidable hospitalization , managed care and the healthcare safety net .
	manualset3
183940	4	414191	7	NULL	NULL	0	NULL	avoidable hospitalization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This analysis examines the affect of 2 healthcare strategies on the rate of avoidable hospitalization , managed care and the healthcare safety net .
	manualset3
183941	5	414191	7	NULL	NULL	0	NULL	care 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This analysis examines the affect of 2 healthcare strategies on the rate of avoidable hospitalization , managed care and the healthcare safety net .
	manualset3
183942	6	414191	7	NULL	NULL	0	NULL	healthcare safety net	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	This analysis examines the affect of 2 healthcare strategies on the rate of avoidable hospitalization , managed care and the healthcare safety net .
	manualset3
183943	1	414192	7	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This analysis provides insights useful for target identification and designing strategies for combination therapy .
	manualset3
183944	2	414192	7	NULL	NULL	0	NULL	target identification	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This analysis provides insights useful for target identification and designing strategies for combination therapy .
	manualset3
183945	3	414192	7	NULL	NULL	0	NULL	designing strategies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This analysis provides insights useful for target identification and designing strategies for combination therapy .
	manualset3
183946	4	414192	7	NULL	NULL	0	NULL	combination therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This analysis provides insights useful for target identification and designing strategies for combination therapy .
	manualset3
183947	1	414193	7	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This analysis provides us with a quantitative picture for intensity and spectral instability in SERRS and SEF within the framework of EM mechanism .
	manualset3
183948	2	414193	7	NULL	NULL	0	NULL	quantitative picture	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	This analysis provides us with a quantitative picture for intensity and spectral instability in SERRS and SEF within the framework of EM mechanism .
	manualset3
183949	3	414193	7	NULL	NULL	0	NULL	intensity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This analysis provides us with a quantitative picture for intensity and spectral instability in SERRS and SEF within the framework of EM mechanism .
	manualset3
183950	4	414193	7	NULL	NULL	0	NULL	spectral instability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This analysis provides us with a quantitative picture for intensity and spectral instability in SERRS and SEF within the framework of EM mechanism .
	manualset3
183951	5	414193	7	NULL	NULL	0	NULL	 SERRS	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This analysis provides us with a quantitative picture for intensity and spectral instability in SERRS and SEF within the framework of EM mechanism .
	manualset3
183952	6	414193	7	NULL	NULL	0	NULL	SEF	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This analysis provides us with a quantitative picture for intensity and spectral instability in SERRS and SEF within the framework of EM mechanism .
	manualset3
183953	7	414193	7	NULL	NULL	0	NULL	framework	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This analysis provides us with a quantitative picture for intensity and spectral instability in SERRS and SEF within the framework of EM mechanism .
	manualset3
183954	8	414193	7	NULL	NULL	0	NULL	EM mechanism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This analysis provides us with a quantitative picture for intensity and spectral instability in SERRS and SEF within the framework of EM mechanism .
	manualset3
183955	1	414194	7	NULL	NULL	0	NULL	enzyme characteristics	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This and other enzyme characteristics indicated that the leaf isozyme corresponded to the type A aleurone alpha-amylase ( low pI group ) .
	manualset3
183956	2	414194	7	NULL	NULL	0	NULL	leaf isozyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This and other enzyme characteristics indicated that the leaf isozyme corresponded to the type A aleurone alpha-amylase ( low pI group ) .
	manualset3
183957	3	414194	7	NULL	NULL	0	NULL	type A aleurone alpha-amylase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This and other enzyme characteristics indicated that the leaf isozyme corresponded to the type A aleurone alpha-amylase ( low pI group ) .
	manualset3
183958	4	414194	7	NULL	NULL	0	NULL	low pI group	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This and other enzyme characteristics indicated that the leaf isozyme corresponded to the type A aleurone alpha-amylase ( low pI group ) .
	manualset3
183959	1	414195	7	NULL	NULL	0	NULL	Additive phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additive phosphorylation of liver glycogen synthase can be observed by the combination of protein kinase C with the former set of kinases but not with the latter .
	manualset3
183960	2	414195	7	NULL	NULL	0	NULL	 liver glycogen synthase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Additive phosphorylation of liver glycogen synthase can be observed by the combination of protein kinase C with the former set of kinases but not with the latter .
	manualset3
183961	3	414195	7	NULL	NULL	0	NULL	combination	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additive phosphorylation of liver glycogen synthase can be observed by the combination of protein kinase C with the former set of kinases but not with the latter .
	manualset3
183962	4	414195	7	NULL	NULL	0	NULL	protein kinase C	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Additive phosphorylation of liver glycogen synthase can be observed by the combination of protein kinase C with the former set of kinases but not with the latter .
	manualset3
183963	5	414195	7	NULL	NULL	0	NULL	former set	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additive phosphorylation of liver glycogen synthase can be observed by the combination of protein kinase C with the former set of kinases but not with the latter .
	manualset3
183964	6	414195	7	NULL	NULL	0	NULL	kinases 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Additive phosphorylation of liver glycogen synthase can be observed by the combination of protein kinase C with the former set of kinases but not with the latter .
	manualset3
183965	1	414196	7	NULL	NULL	0	NULL	antibiotic	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	This antibiotic displays two major characteristics : a very long serum half-life and a good tissue penetration .
	manualset3
183966	2	414196	7	NULL	NULL	NULL	NULL	two major characteristics	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This antibiotic displays two major characteristics : a very long serum half-life and a good tissue penetration .
	manualset3
183967	3	414196	7	NULL	NULL	0	NULL	very long serum half-life	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	This antibiotic displays two major characteristics : a very long serum half-life and a good tissue penetration .
	manualset3
183968	4	414196	7	NULL	NULL	0	NULL	good tissue penetration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This antibiotic displays two major characteristics : a very long serum half-life and a good tissue penetration .
	manualset3
183969	1	414197	7	NULL	NULL	0	NULL	antiserum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This antiserum also reacted with tumor structures in 18/18 pancreatic adenocarcinomas as well as with pancreatic acini in the vicinity of tumor .
	manualset3
183970	2	414197	7	NULL	NULL	0	NULL	tumor structures 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This antiserum also reacted with tumor structures in 18/18 pancreatic adenocarcinomas as well as with pancreatic acini in the vicinity of tumor .
	manualset3
183971	3	414197	7	NULL	NULL	0	NULL	18/18 pancreatic adenocarcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This antiserum also reacted with tumor structures in 18/18 pancreatic adenocarcinomas as well as with pancreatic acini in the vicinity of tumor .
	manualset3
183972	4	414197	7	NULL	NULL	0	NULL	pancreatic acini	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	This antiserum also reacted with tumor structures in 18/18 pancreatic adenocarcinomas as well as with pancreatic acini in the vicinity of tumor .
	manualset3
183973	5	414197	7	NULL	NULL	0	NULL	vicinity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This antiserum also reacted with tumor structures in 18/18 pancreatic adenocarcinomas as well as with pancreatic acini in the vicinity of tumor .
	manualset3
183974	6	414197	7	NULL	NULL	0	NULL	tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This antiserum also reacted with tumor structures in 18/18 pancreatic adenocarcinomas as well as with pancreatic acini in the vicinity of tumor .
	manualset3
183975	1	414198	7	NULL	NULL	0	NULL	apoptotic mechanism 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This apoptotic mechanism was mediated by a chondroitin sulfate proteoglycan , since treating cells with chondroitin sulfate or chondroitinase reversed the apoptotic cell shape changes .
	manualset3
183976	2	414198	7	NULL	NULL	NULL	NULL	chondroitin sulfate proteoglycan	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This apoptotic mechanism was mediated by a chondroitin sulfate proteoglycan , since treating cells with chondroitin sulfate or chondroitinase reversed the apoptotic cell shape changes .
	manualset3
183977	3	414198	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	This apoptotic mechanism was mediated by a chondroitin sulfate proteoglycan , since treating cells with chondroitin sulfate or chondroitinase reversed the apoptotic cell shape changes .
	manualset3
183978	4	414198	7	NULL	NULL	0	NULL	chondroitin sulfate 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This apoptotic mechanism was mediated by a chondroitin sulfate proteoglycan , since treating cells with chondroitin sulfate or chondroitinase reversed the apoptotic cell shape changes .
	manualset3
183979	5	414198	7	NULL	NULL	0	NULL	chondroitinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This apoptotic mechanism was mediated by a chondroitin sulfate proteoglycan , since treating cells with chondroitin sulfate or chondroitinase reversed the apoptotic cell shape changes .
	manualset3
183980	6	414198	7	NULL	NULL	0	NULL	apoptotic cell shape changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This apoptotic mechanism was mediated by a chondroitin sulfate proteoglycan , since treating cells with chondroitin sulfate or chondroitinase reversed the apoptotic cell shape changes .
	manualset3
183981	1	414199	7	NULL	NULL	0	NULL	first-row metallabenzenes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This appears to be particularly true of first-row and second-row metallabenzenes , where the metal-carbon bond strengths are weaker .
	manualset3
183982	2	414199	7	NULL	NULL	0	NULL	second-row metallabenzenes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This appears to be particularly true of first-row and second-row metallabenzenes , where the metal-carbon bond strengths are weaker .
	manualset3
183983	3	414199	7	NULL	NULL	NULL	NULL	metal-carbon bond strengths	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This appears to be particularly true of first-row and second-row metallabenzenes , where the metal-carbon bond strengths are weaker .
	manualset3
183984	1	414200	7	NULL	NULL	0	NULL	first report 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This appears to be the first report of serious muscle contracture after cosmetic radiofrequency volume reduction requiring extensive rehabilitation management .
	manualset3
183985	2	414200	7	NULL	NULL	0	NULL	serious muscle contracture	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This appears to be the first report of serious muscle contracture after cosmetic radiofrequency volume reduction requiring extensive rehabilitation management .
	manualset3
183986	3	414200	7	NULL	NULL	0	NULL	cosmetic radiofrequency volume reduction	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This appears to be the first report of serious muscle contracture after cosmetic radiofrequency volume reduction requiring extensive rehabilitation management .
	manualset3
183987	4	414200	7	NULL	NULL	0	NULL	extensive rehabilitation management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This appears to be the first report of serious muscle contracture after cosmetic radiofrequency volume reduction requiring extensive rehabilitation management .
	manualset3
183988	1	414201	7	NULL	NULL	0	NULL	approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This approach demonstrated that Tyr-192 is the major chlorination site in apoA-I in both plasma and lesion HDL of humans .
	manualset3
183989	2	414201	7	NULL	NULL	0	NULL	Tyr-192	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	This approach demonstrated that Tyr-192 is the major chlorination site in apoA-I in both plasma and lesion HDL of humans .
	manualset3
183990	3	414201	7	NULL	NULL	0	NULL	major chlorination site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	This approach demonstrated that Tyr-192 is the major chlorination site in apoA-I in both plasma and lesion HDL of humans .
	manualset3
183991	4	414201	7	NULL	NULL	0	NULL	apoA-I	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This approach demonstrated that Tyr-192 is the major chlorination site in apoA-I in both plasma and lesion HDL of humans .
	manualset3
183992	5	414201	7	NULL	NULL	0	NULL	plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This approach demonstrated that Tyr-192 is the major chlorination site in apoA-I in both plasma and lesion HDL of humans .
	manualset3
183993	6	414201	7	NULL	NULL	0	NULL	lesion HDL	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This approach demonstrated that Tyr-192 is the major chlorination site in apoA-I in both plasma and lesion HDL of humans .
	manualset3
183994	7	414201	7	NULL	NULL	0	NULL	humans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	This approach demonstrated that Tyr-192 is the major chlorination site in apoA-I in both plasma and lesion HDL of humans .
	manualset3
183995	1	414202	7	NULL	NULL	0	NULL	approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This approach enabled the use of the Zimm plots in order to determine the radii of gyration and the radii of spherical particles .
	manualset3
183996	2	414202	7	NULL	NULL	0	NULL	Zimm plots 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This approach enabled the use of the Zimm plots in order to determine the radii of gyration and the radii of spherical particles .
	manualset3
183997	3	414202	7	NULL	NULL	0	NULL	radii of gyration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This approach enabled the use of the Zimm plots in order to determine the radii of gyration and the radii of spherical particles .
	manualset3
183998	4	414202	7	NULL	NULL	0	NULL	 radii of spherical particles 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This approach enabled the use of the Zimm plots in order to determine the radii of gyration and the radii of spherical particles .
	manualset3
183999	1	414203	7	NULL	NULL	0	NULL	approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This approach is informative for the study of both recombinant and native chromatin complexes consisting either of histone subunits alone or in association with accessory proteins , in this case histone chaperones .
	manualset3
184000	2	414203	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This approach is informative for the study of both recombinant and native chromatin complexes consisting either of histone subunits alone or in association with accessory proteins , in this case histone chaperones .
	manualset3
184001	3	414203	7	NULL	NULL	0	NULL	recombinant chromatin complexes	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	This approach is informative for the study of both recombinant and native chromatin complexes consisting either of histone subunits alone or in association with accessory proteins , in this case histone chaperones .
	manualset3
184002	4	414203	7	NULL	NULL	0	NULL	native chromatin complexes	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	This approach is informative for the study of both recombinant and native chromatin complexes consisting either of histone subunits alone or in association with accessory proteins , in this case histone chaperones .
	manualset3
184003	5	414203	7	NULL	NULL	0	NULL	histone subunits	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This approach is informative for the study of both recombinant and native chromatin complexes consisting either of histone subunits alone or in association with accessory proteins , in this case histone chaperones .
	manualset3
184004	6	414203	7	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	This approach is informative for the study of both recombinant and native chromatin complexes consisting either of histone subunits alone or in association with accessory proteins , in this case histone chaperones .
	manualset3
184005	7	414203	7	NULL	NULL	0	NULL	accessory proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This approach is informative for the study of both recombinant and native chromatin complexes consisting either of histone subunits alone or in association with accessory proteins , in this case histone chaperones .
	manualset3
184006	8	414203	7	NULL	NULL	0	NULL	histone chaperones	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This approach is informative for the study of both recombinant and native chromatin complexes consisting either of histone subunits alone or in association with accessory proteins , in this case histone chaperones .
	manualset3
184007	1	414204	7	NULL	NULL	0	NULL	 article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article , second in a series of three articles focusing on Kernberg 's ( 1975 , 1984 ) psychostructural diagnosis of personality organization , examines Rorschach contributions to the description and diagnosis of borderline personality organization .
	manualset3
184008	2	414204	7	NULL	NULL	0	NULL	series	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article , second in a series of three articles focusing on Kernberg 's ( 1975 , 1984 ) psychostructural diagnosis of personality organization , examines Rorschach contributions to the description and diagnosis of borderline personality organization .
	manualset3
184009	3	414204	7	NULL	NULL	0	NULL	three articles	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article , second in a series of three articles focusing on Kernberg 's ( 1975 , 1984 ) psychostructural diagnosis of personality organization , examines Rorschach contributions to the description and diagnosis of borderline personality organization .
	manualset3
184010	4	414204	7	NULL	NULL	0	NULL	Kernberg 's ( 1975 , 1984 ) psychostructural diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This article , second in a series of three articles focusing on Kernberg 's ( 1975 , 1984 ) psychostructural diagnosis of personality organization , examines Rorschach contributions to the description and diagnosis of borderline personality organization .
	manualset3
184011	5	414204	7	NULL	NULL	0	NULL	personality organization	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	This article , second in a series of three articles focusing on Kernberg 's ( 1975 , 1984 ) psychostructural diagnosis of personality organization , examines Rorschach contributions to the description and diagnosis of borderline personality organization .
	manualset3
184012	6	414204	7	NULL	NULL	0	NULL	Rorschach contributions	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article , second in a series of three articles focusing on Kernberg 's ( 1975 , 1984 ) psychostructural diagnosis of personality organization , examines Rorschach contributions to the description and diagnosis of borderline personality organization .
	manualset3
184013	7	414204	7	NULL	NULL	0	NULL	description 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article , second in a series of three articles focusing on Kernberg 's ( 1975 , 1984 ) psychostructural diagnosis of personality organization , examines Rorschach contributions to the description and diagnosis of borderline personality organization .
	manualset3
184014	8	414204	7	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This article , second in a series of three articles focusing on Kernberg 's ( 1975 , 1984 ) psychostructural diagnosis of personality organization , examines Rorschach contributions to the description and diagnosis of borderline personality organization .
	manualset3
184015	9	414204	7	NULL	NULL	0	NULL	borderline personality organization	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	This article , second in a series of three articles focusing on Kernberg 's ( 1975 , 1984 ) psychostructural diagnosis of personality organization , examines Rorschach contributions to the description and diagnosis of borderline personality organization .
	manualset3
184016	1	414205	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article argues for the importance of Europe 's continental empires , Habsburg and Romanov , to the emergence of a physical-dynamical model of the global climate before World War I. It begins to identify a set of questions and methods that were distinctive of climatology as a continental-imperial science of `` regionalization '' with a global vision .
	manualset3
184017	2	414205	7	NULL	NULL	0	NULL	importance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article argues for the importance of Europe 's continental empires , Habsburg and Romanov , to the emergence of a physical-dynamical model of the global climate before World War I. It begins to identify a set of questions and methods that were distinctive of climatology as a continental-imperial science of `` regionalization '' with a global vision .
	manualset3
184018	3	414205	7	NULL	NULL	0	NULL	Europe 's continental empires	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article argues for the importance of Europe 's continental empires , Habsburg and Romanov , to the emergence of a physical-dynamical model of the global climate before World War I. It begins to identify a set of questions and methods that were distinctive of climatology as a continental-imperial science of `` regionalization '' with a global vision .
	manualset3
184019	4	414205	7	NULL	NULL	0	NULL	Habsburg	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	This article argues for the importance of Europe 's continental empires , Habsburg and Romanov , to the emergence of a physical-dynamical model of the global climate before World War I. It begins to identify a set of questions and methods that were distinctive of climatology as a continental-imperial science of `` regionalization '' with a global vision .
	manualset3
184020	5	414205	7	NULL	NULL	0	NULL	Romanov	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	This article argues for the importance of Europe 's continental empires , Habsburg and Romanov , to the emergence of a physical-dynamical model of the global climate before World War I. It begins to identify a set of questions and methods that were distinctive of climatology as a continental-imperial science of `` regionalization '' with a global vision .
	manualset3
184021	6	414205	7	NULL	NULL	0	NULL	emergence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article argues for the importance of Europe 's continental empires , Habsburg and Romanov , to the emergence of a physical-dynamical model of the global climate before World War I. It begins to identify a set of questions and methods that were distinctive of climatology as a continental-imperial science of `` regionalization '' with a global vision .
	manualset3
184022	7	414205	7	NULL	NULL	0	NULL	physical-dynamical model 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	This article argues for the importance of Europe 's continental empires , Habsburg and Romanov , to the emergence of a physical-dynamical model of the global climate before World War I. It begins to identify a set of questions and methods that were distinctive of climatology as a continental-imperial science of `` regionalization '' with a global vision .
	manualset3
184023	8	414205	7	NULL	NULL	0	NULL	global climate 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	This article argues for the importance of Europe 's continental empires , Habsburg and Romanov , to the emergence of a physical-dynamical model of the global climate before World War I. It begins to identify a set of questions and methods that were distinctive of climatology as a continental-imperial science of `` regionalization '' with a global vision .
	manualset3
184024	9	414205	7	NULL	NULL	0	NULL	World War I	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article argues for the importance of Europe 's continental empires , Habsburg and Romanov , to the emergence of a physical-dynamical model of the global climate before World War I. It begins to identify a set of questions and methods that were distinctive of climatology as a continental-imperial science of `` regionalization '' with a global vision .
	manualset3
184025	10	414205	7	NULL	NULL	0	NULL	set	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article argues for the importance of Europe 's continental empires , Habsburg and Romanov , to the emergence of a physical-dynamical model of the global climate before World War I. It begins to identify a set of questions and methods that were distinctive of climatology as a continental-imperial science of `` regionalization '' with a global vision .
	manualset3
184026	11	414205	7	NULL	NULL	0	NULL	questions	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article argues for the importance of Europe 's continental empires , Habsburg and Romanov , to the emergence of a physical-dynamical model of the global climate before World War I. It begins to identify a set of questions and methods that were distinctive of climatology as a continental-imperial science of `` regionalization '' with a global vision .
	manualset3
184027	12	414205	7	NULL	NULL	0	NULL	methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article argues for the importance of Europe 's continental empires , Habsburg and Romanov , to the emergence of a physical-dynamical model of the global climate before World War I. It begins to identify a set of questions and methods that were distinctive of climatology as a continental-imperial science of `` regionalization '' with a global vision .
	manualset3
184028	13	414205	7	NULL	NULL	0	NULL	climatology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This article argues for the importance of Europe 's continental empires , Habsburg and Romanov , to the emergence of a physical-dynamical model of the global climate before World War I. It begins to identify a set of questions and methods that were distinctive of climatology as a continental-imperial science of `` regionalization '' with a global vision .
	manualset3
184029	14	414205	7	NULL	NULL	0	NULL	continental-imperial science	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This article argues for the importance of Europe 's continental empires , Habsburg and Romanov , to the emergence of a physical-dynamical model of the global climate before World War I. It begins to identify a set of questions and methods that were distinctive of climatology as a continental-imperial science of `` regionalization '' with a global vision .
	manualset3
184030	15	414205	7	NULL	NULL	0	NULL	regionalization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article argues for the importance of Europe 's continental empires , Habsburg and Romanov , to the emergence of a physical-dynamical model of the global climate before World War I. It begins to identify a set of questions and methods that were distinctive of climatology as a continental-imperial science of `` regionalization '' with a global vision .
	manualset3
184031	16	414205	7	NULL	NULL	0	NULL	global vision 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article argues for the importance of Europe 's continental empires , Habsburg and Romanov , to the emergence of a physical-dynamical model of the global climate before World War I. It begins to identify a set of questions and methods that were distinctive of climatology as a continental-imperial science of `` regionalization '' with a global vision .
	manualset3
184032	1	414206	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article compares , describes , and analyzes case management in six program categories : ( a ) for persons suffering from chronic mental illness ; ( b ) in child welfare ; ( c ) in community-based long-term care ; ( d ) for children and adolescents suffering from severe emotional disturbance ; ( e ) for individuals experiencing substance abuse problems ; and ( f ) in the public welfare system .
	manualset3
184033	2	414206	7	NULL	NULL	0	NULL	case management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article compares , describes , and analyzes case management in six program categories : ( a ) for persons suffering from chronic mental illness ; ( b ) in child welfare ; ( c ) in community-based long-term care ; ( d ) for children and adolescents suffering from severe emotional disturbance ; ( e ) for individuals experiencing substance abuse problems ; and ( f ) in the public welfare system .
	manualset3
184034	3	414206	7	NULL	NULL	0	NULL	 six program categories	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article compares , describes , and analyzes case management in six program categories : ( a ) for persons suffering from chronic mental illness ; ( b ) in child welfare ; ( c ) in community-based long-term care ; ( d ) for children and adolescents suffering from severe emotional disturbance ; ( e ) for individuals experiencing substance abuse problems ; and ( f ) in the public welfare system .
	manualset3
184035	4	414206	7	NULL	NULL	0	NULL	persons	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This article compares , describes , and analyzes case management in six program categories : ( a ) for persons suffering from chronic mental illness ; ( b ) in child welfare ; ( c ) in community-based long-term care ; ( d ) for children and adolescents suffering from severe emotional disturbance ; ( e ) for individuals experiencing substance abuse problems ; and ( f ) in the public welfare system .
	manualset3
184036	5	414206	7	NULL	NULL	0	NULL	chronic mental illness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article compares , describes , and analyzes case management in six program categories : ( a ) for persons suffering from chronic mental illness ; ( b ) in child welfare ; ( c ) in community-based long-term care ; ( d ) for children and adolescents suffering from severe emotional disturbance ; ( e ) for individuals experiencing substance abuse problems ; and ( f ) in the public welfare system .
	manualset3
184037	6	414206	7	NULL	NULL	0	NULL	child welfare	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article compares , describes , and analyzes case management in six program categories : ( a ) for persons suffering from chronic mental illness ; ( b ) in child welfare ; ( c ) in community-based long-term care ; ( d ) for children and adolescents suffering from severe emotional disturbance ; ( e ) for individuals experiencing substance abuse problems ; and ( f ) in the public welfare system .
	manualset3
184038	7	414206	7	NULL	NULL	0	NULL	community-based long-term care	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	This article compares , describes , and analyzes case management in six program categories : ( a ) for persons suffering from chronic mental illness ; ( b ) in child welfare ; ( c ) in community-based long-term care ; ( d ) for children and adolescents suffering from severe emotional disturbance ; ( e ) for individuals experiencing substance abuse problems ; and ( f ) in the public welfare system .
	manualset3
184039	8	414206	7	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This article compares , describes , and analyzes case management in six program categories : ( a ) for persons suffering from chronic mental illness ; ( b ) in child welfare ; ( c ) in community-based long-term care ; ( d ) for children and adolescents suffering from severe emotional disturbance ; ( e ) for individuals experiencing substance abuse problems ; and ( f ) in the public welfare system .
	manualset3
184040	9	414206	7	NULL	NULL	0	NULL	adolescents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This article compares , describes , and analyzes case management in six program categories : ( a ) for persons suffering from chronic mental illness ; ( b ) in child welfare ; ( c ) in community-based long-term care ; ( d ) for children and adolescents suffering from severe emotional disturbance ; ( e ) for individuals experiencing substance abuse problems ; and ( f ) in the public welfare system .
	manualset3
184041	10	414206	7	NULL	NULL	0	NULL	severe emotional disturbance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article compares , describes , and analyzes case management in six program categories : ( a ) for persons suffering from chronic mental illness ; ( b ) in child welfare ; ( c ) in community-based long-term care ; ( d ) for children and adolescents suffering from severe emotional disturbance ; ( e ) for individuals experiencing substance abuse problems ; and ( f ) in the public welfare system .
	manualset3
184042	11	414206	7	NULL	NULL	0	NULL	individuals	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	This article compares , describes , and analyzes case management in six program categories : ( a ) for persons suffering from chronic mental illness ; ( b ) in child welfare ; ( c ) in community-based long-term care ; ( d ) for children and adolescents suffering from severe emotional disturbance ; ( e ) for individuals experiencing substance abuse problems ; and ( f ) in the public welfare system .
	manualset3
184043	12	414206	7	NULL	NULL	0	NULL	substance abuse problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article compares , describes , and analyzes case management in six program categories : ( a ) for persons suffering from chronic mental illness ; ( b ) in child welfare ; ( c ) in community-based long-term care ; ( d ) for children and adolescents suffering from severe emotional disturbance ; ( e ) for individuals experiencing substance abuse problems ; and ( f ) in the public welfare system .
	manualset3
184044	13	414206	7	NULL	NULL	0	NULL	public welfare system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	This article compares , describes , and analyzes case management in six program categories : ( a ) for persons suffering from chronic mental illness ; ( b ) in child welfare ; ( c ) in community-based long-term care ; ( d ) for children and adolescents suffering from severe emotional disturbance ; ( e ) for individuals experiencing substance abuse problems ; and ( f ) in the public welfare system .
	manualset3
184045	1	414207	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes CRGs , their underlying concepts , development efforts , their relevance to biosecurity and bioterrorism , and future research issues in the use of technology to facilitate community response .
	manualset3
184046	2	414207	7	NULL	NULL	0	NULL	CRGs	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes CRGs , their underlying concepts , development efforts , their relevance to biosecurity and bioterrorism , and future research issues in the use of technology to facilitate community response .
	manualset3
184047	3	414207	7	NULL	NULL	0	NULL	concepts	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes CRGs , their underlying concepts , development efforts , their relevance to biosecurity and bioterrorism , and future research issues in the use of technology to facilitate community response .
	manualset3
184048	4	414207	7	NULL	NULL	0	NULL	development efforts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes CRGs , their underlying concepts , development efforts , their relevance to biosecurity and bioterrorism , and future research issues in the use of technology to facilitate community response .
	manualset3
184049	5	414207	7	NULL	NULL	0	NULL	biosecurity	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes CRGs , their underlying concepts , development efforts , their relevance to biosecurity and bioterrorism , and future research issues in the use of technology to facilitate community response .
	manualset3
184050	6	414207	7	NULL	NULL	0	NULL	bioterrorism	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes CRGs , their underlying concepts , development efforts , their relevance to biosecurity and bioterrorism , and future research issues in the use of technology to facilitate community response .
	manualset3
184051	7	414207	7	NULL	NULL	0	NULL	future research issues	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes CRGs , their underlying concepts , development efforts , their relevance to biosecurity and bioterrorism , and future research issues in the use of technology to facilitate community response .
	manualset3
184052	8	414207	7	NULL	NULL	0	NULL	technology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes CRGs , their underlying concepts , development efforts , their relevance to biosecurity and bioterrorism , and future research issues in the use of technology to facilitate community response .
	manualset3
184053	9	414207	7	NULL	NULL	0	NULL	community response	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes CRGs , their underlying concepts , development efforts , their relevance to biosecurity and bioterrorism , and future research issues in the use of technology to facilitate community response .
	manualset3
184054	1	414208	7	NULL	NULL	0	NULL	article 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes a method to workup patients with solid submucosal lesions of the larynx to diagnose a paraganglioma without a biopsy .
	manualset3
184055	2	414208	7	NULL	NULL	0	NULL	 method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes a method to workup patients with solid submucosal lesions of the larynx to diagnose a paraganglioma without a biopsy .
	manualset3
184056	3	414208	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes a method to workup patients with solid submucosal lesions of the larynx to diagnose a paraganglioma without a biopsy .
	manualset3
184057	4	414208	7	NULL	NULL	0	NULL	solid submucosal lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes a method to workup patients with solid submucosal lesions of the larynx to diagnose a paraganglioma without a biopsy .
	manualset3
184058	5	414208	7	NULL	NULL	0	NULL	larynx	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes a method to workup patients with solid submucosal lesions of the larynx to diagnose a paraganglioma without a biopsy .
	manualset3
184059	6	414208	7	NULL	NULL	0	NULL	paraganglioma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes a method to workup patients with solid submucosal lesions of the larynx to diagnose a paraganglioma without a biopsy .
	manualset3
184060	7	414208	7	NULL	NULL	0	NULL	biopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes a method to workup patients with solid submucosal lesions of the larynx to diagnose a paraganglioma without a biopsy .
	manualset3
184061	1	414209	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes a project for the integration into work of unemployed female immigrants by means of two parallel programs : ( 1 ) workshop for job-seeking skills ; ( 2 ) establishment and operation of a self-help group .
	manualset3
184062	2	414209	7	NULL	NULL	NULL	NULL	project	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This article describes a project for the integration into work of unemployed female immigrants by means of two parallel programs : ( 1 ) workshop for job-seeking skills ; ( 2 ) establishment and operation of a self-help group .
	manualset3
184063	3	414209	7	NULL	NULL	0	NULL	integration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes a project for the integration into work of unemployed female immigrants by means of two parallel programs : ( 1 ) workshop for job-seeking skills ; ( 2 ) establishment and operation of a self-help group .
	manualset3
184064	4	414209	7	NULL	NULL	0	NULL	work	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes a project for the integration into work of unemployed female immigrants by means of two parallel programs : ( 1 ) workshop for job-seeking skills ; ( 2 ) establishment and operation of a self-help group .
	manualset3
184065	5	414209	7	NULL	NULL	0	NULL	unemployed female immigrants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes a project for the integration into work of unemployed female immigrants by means of two parallel programs : ( 1 ) workshop for job-seeking skills ; ( 2 ) establishment and operation of a self-help group .
	manualset3
184066	6	414209	7	NULL	NULL	0	NULL	two parallel programs	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes a project for the integration into work of unemployed female immigrants by means of two parallel programs : ( 1 ) workshop for job-seeking skills ; ( 2 ) establishment and operation of a self-help group .
	manualset3
184067	7	414209	7	NULL	NULL	0	NULL	 workshop	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes a project for the integration into work of unemployed female immigrants by means of two parallel programs : ( 1 ) workshop for job-seeking skills ; ( 2 ) establishment and operation of a self-help group .
	manualset3
184068	8	414209	7	NULL	NULL	0	NULL	job-seeking skills	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes a project for the integration into work of unemployed female immigrants by means of two parallel programs : ( 1 ) workshop for job-seeking skills ; ( 2 ) establishment and operation of a self-help group .
	manualset3
184069	9	414209	7	NULL	NULL	0	NULL	establishment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes a project for the integration into work of unemployed female immigrants by means of two parallel programs : ( 1 ) workshop for job-seeking skills ; ( 2 ) establishment and operation of a self-help group .
	manualset3
184070	10	414209	7	NULL	NULL	0	NULL	operation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes a project for the integration into work of unemployed female immigrants by means of two parallel programs : ( 1 ) workshop for job-seeking skills ; ( 2 ) establishment and operation of a self-help group .
	manualset3
184071	11	414209	7	NULL	NULL	0	NULL	self-help group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes a project for the integration into work of unemployed female immigrants by means of two parallel programs : ( 1 ) workshop for job-seeking skills ; ( 2 ) establishment and operation of a self-help group .
	manualset3
184072	1	414210	7	NULL	NULL	0	NULL	Adenocarcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenocarcinoma of the uterine cervix with choriocarcinomatous metastasis .
	manualset3
184073	2	414210	7	NULL	NULL	0	NULL	uterine cervix	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenocarcinoma of the uterine cervix with choriocarcinomatous metastasis .
	manualset3
184074	3	414210	7	NULL	NULL	0	NULL	choriocarcinomatous metastasis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenocarcinoma of the uterine cervix with choriocarcinomatous metastasis .
	manualset3
184075	1	414211	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes pathophysiological mechanisms involved in the defective uteroplacental vascularization leading to placental and endothelial dysfunction .
	manualset3
184076	2	414211	7	NULL	NULL	0	NULL	pathophysiological mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes pathophysiological mechanisms involved in the defective uteroplacental vascularization leading to placental and endothelial dysfunction .
	manualset3
184077	3	414211	7	NULL	NULL	0	NULL	defective uteroplacental vascularization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes pathophysiological mechanisms involved in the defective uteroplacental vascularization leading to placental and endothelial dysfunction .
	manualset3
184078	4	414211	7	NULL	NULL	0	NULL	placental dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes pathophysiological mechanisms involved in the defective uteroplacental vascularization leading to placental and endothelial dysfunction .
	manualset3
184079	5	414211	7	NULL	NULL	0	NULL	endothelial dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes pathophysiological mechanisms involved in the defective uteroplacental vascularization leading to placental and endothelial dysfunction .
	manualset3
184080	1	414212	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes the body of work in this field where comparative proteomics methods have been used for the discovery of putative biomarkers associated with radiotherapy resistance .
	manualset3
184081	2	414212	7	NULL	NULL	0	NULL	body of work 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes the body of work in this field where comparative proteomics methods have been used for the discovery of putative biomarkers associated with radiotherapy resistance .
	manualset3
184082	3	414212	7	NULL	NULL	0	NULL	field	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes the body of work in this field where comparative proteomics methods have been used for the discovery of putative biomarkers associated with radiotherapy resistance .
	manualset3
184083	4	414212	7	NULL	NULL	0	NULL	comparative proteomics methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes the body of work in this field where comparative proteomics methods have been used for the discovery of putative biomarkers associated with radiotherapy resistance .
	manualset3
184084	5	414212	7	NULL	NULL	0	NULL	discovery	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes the body of work in this field where comparative proteomics methods have been used for the discovery of putative biomarkers associated with radiotherapy resistance .
	manualset3
184085	6	414212	7	NULL	NULL	0	NULL	putative biomarkers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes the body of work in this field where comparative proteomics methods have been used for the discovery of putative biomarkers associated with radiotherapy resistance .
	manualset3
184086	7	414212	7	NULL	NULL	0	NULL	radiotherapy resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes the body of work in this field where comparative proteomics methods have been used for the discovery of putative biomarkers associated with radiotherapy resistance .
	manualset3
184087	1	414213	7	NULL	NULL	0	NULL	 article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes the concept of social justice advocacy as currently reflected in professional codes and nursing literature and contrasts this with the individual patient-nurse advocacy model , which continues to dominate in nursing practice today .
	manualset3
184088	2	414213	7	NULL	NULL	0	NULL	concept 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes the concept of social justice advocacy as currently reflected in professional codes and nursing literature and contrasts this with the individual patient-nurse advocacy model , which continues to dominate in nursing practice today .
	manualset3
184089	3	414213	7	NULL	NULL	0	NULL	social justice advocacy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes the concept of social justice advocacy as currently reflected in professional codes and nursing literature and contrasts this with the individual patient-nurse advocacy model , which continues to dominate in nursing practice today .
	manualset3
184090	4	414213	7	NULL	NULL	0	NULL	 professional codes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes the concept of social justice advocacy as currently reflected in professional codes and nursing literature and contrasts this with the individual patient-nurse advocacy model , which continues to dominate in nursing practice today .
	manualset3
184091	5	414213	7	NULL	NULL	0	NULL	nursing literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes the concept of social justice advocacy as currently reflected in professional codes and nursing literature and contrasts this with the individual patient-nurse advocacy model , which continues to dominate in nursing practice today .
	manualset3
184092	6	414213	7	NULL	NULL	0	NULL	individual patient-nurse advocacy model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes the concept of social justice advocacy as currently reflected in professional codes and nursing literature and contrasts this with the individual patient-nurse advocacy model , which continues to dominate in nursing practice today .
	manualset3
184093	7	414213	7	NULL	NULL	0	NULL	nursing practice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes the concept of social justice advocacy as currently reflected in professional codes and nursing literature and contrasts this with the individual patient-nurse advocacy model , which continues to dominate in nursing practice today .
	manualset3
184094	8	414213	7	NULL	NULL	0	NULL	today	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes the concept of social justice advocacy as currently reflected in professional codes and nursing literature and contrasts this with the individual patient-nurse advocacy model , which continues to dominate in nursing practice today .
	manualset3
184095	1	414214	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes the current status of , and central issues in , efforts to create models for health care credentialing of chiropractors , acupuncturists , naturopaths , massage therapists , and other CAM practitioners .
	manualset3
184096	2	414214	7	NULL	NULL	0	NULL	current status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes the current status of , and central issues in , efforts to create models for health care credentialing of chiropractors , acupuncturists , naturopaths , massage therapists , and other CAM practitioners .
	manualset3
184097	3	414214	7	NULL	NULL	0	NULL	central issues	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes the current status of , and central issues in , efforts to create models for health care credentialing of chiropractors , acupuncturists , naturopaths , massage therapists , and other CAM practitioners .
	manualset3
184098	4	414214	7	NULL	NULL	NULL	NULL	 models	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This article describes the current status of , and central issues in , efforts to create models for health care credentialing of chiropractors , acupuncturists , naturopaths , massage therapists , and other CAM practitioners .
	manualset3
184099	5	414214	7	NULL	NULL	0	NULL	health care credentialing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes the current status of , and central issues in , efforts to create models for health care credentialing of chiropractors , acupuncturists , naturopaths , massage therapists , and other CAM practitioners .
	manualset3
184100	6	414214	7	NULL	NULL	0	NULL	chiropractors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes the current status of , and central issues in , efforts to create models for health care credentialing of chiropractors , acupuncturists , naturopaths , massage therapists , and other CAM practitioners .
	manualset3
184101	7	414214	7	NULL	NULL	0	NULL	acupuncturists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes the current status of , and central issues in , efforts to create models for health care credentialing of chiropractors , acupuncturists , naturopaths , massage therapists , and other CAM practitioners .
	manualset3
184102	8	414214	7	NULL	NULL	0	NULL	naturopaths	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes the current status of , and central issues in , efforts to create models for health care credentialing of chiropractors , acupuncturists , naturopaths , massage therapists , and other CAM practitioners .
	manualset3
184103	9	414214	7	NULL	NULL	0	NULL	massage therapists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes the current status of , and central issues in , efforts to create models for health care credentialing of chiropractors , acupuncturists , naturopaths , massage therapists , and other CAM practitioners .
	manualset3
184104	10	414214	7	NULL	NULL	0	NULL	CAM practitioners	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This article describes the current status of , and central issues in , efforts to create models for health care credentialing of chiropractors , acupuncturists , naturopaths , massage therapists , and other CAM practitioners .
	manualset3
184105	1	414215	7	NULL	NULL	0	NULL	 article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article discusses the many uses of transesophageal echocardiography in this population , in the outpatient setting , in the peri-operative period , and in the cardiac catheterization laboratory .
	manualset3
184106	2	414215	7	NULL	NULL	NULL	NULL	transesophageal echocardiography	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This article discusses the many uses of transesophageal echocardiography in this population , in the outpatient setting , in the peri-operative period , and in the cardiac catheterization laboratory .
	manualset3
184107	3	414215	7	NULL	NULL	0	NULL	population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This article discusses the many uses of transesophageal echocardiography in this population , in the outpatient setting , in the peri-operative period , and in the cardiac catheterization laboratory .
	manualset3
184108	4	414215	7	NULL	NULL	0	NULL	outpatient setting	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This article discusses the many uses of transesophageal echocardiography in this population , in the outpatient setting , in the peri-operative period , and in the cardiac catheterization laboratory .
	manualset3
184109	5	414215	7	NULL	NULL	0	NULL	peri-operative period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	This article discusses the many uses of transesophageal echocardiography in this population , in the outpatient setting , in the peri-operative period , and in the cardiac catheterization laboratory .
	manualset3
184110	6	414215	7	NULL	NULL	0	NULL	cardiac catheterization laboratory	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	This article discusses the many uses of transesophageal echocardiography in this population , in the outpatient setting , in the peri-operative period , and in the cardiac catheterization laboratory .
	manualset3
184111	1	414216	7	NULL	NULL	0	NULL	Adenoidectomy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenoidectomy was found to be more hemorrhagic than adenotonsillectomy , in particular in the presence of a large clump of adenoids and in autumn or winter .
	manualset3
184112	2	414216	7	NULL	NULL	0	NULL	hemorrhagic	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenoidectomy was found to be more hemorrhagic than adenotonsillectomy , in particular in the presence of a large clump of adenoids and in autumn or winter .
	manualset3
184113	3	414216	7	NULL	NULL	0	NULL	adenotonsillectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenoidectomy was found to be more hemorrhagic than adenotonsillectomy , in particular in the presence of a large clump of adenoids and in autumn or winter .
	manualset3
184114	4	414216	7	NULL	NULL	0	NULL	presence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenoidectomy was found to be more hemorrhagic than adenotonsillectomy , in particular in the presence of a large clump of adenoids and in autumn or winter .
	manualset3
184115	5	414216	7	NULL	NULL	0	NULL	large clump	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenoidectomy was found to be more hemorrhagic than adenotonsillectomy , in particular in the presence of a large clump of adenoids and in autumn or winter .
	manualset3
184116	6	414216	7	NULL	NULL	0	NULL	adenoids	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenoidectomy was found to be more hemorrhagic than adenotonsillectomy , in particular in the presence of a large clump of adenoids and in autumn or winter .
	manualset3
184117	7	414216	7	NULL	NULL	0	NULL	autumn 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenoidectomy was found to be more hemorrhagic than adenotonsillectomy , in particular in the presence of a large clump of adenoids and in autumn or winter .
	manualset3
184118	8	414216	7	NULL	NULL	0	NULL	winter	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenoidectomy was found to be more hemorrhagic than adenotonsillectomy , in particular in the presence of a large clump of adenoids and in autumn or winter .
	manualset3
184119	1	414217	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines postulated mechanisms for cerebral injury from cardiac surgery .
	manualset3
184120	2	414217	7	NULL	NULL	0	NULL	postulated mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines postulated mechanisms for cerebral injury from cardiac surgery .
	manualset3
184121	3	414217	7	NULL	NULL	0	NULL	cerebral injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines postulated mechanisms for cerebral injury from cardiac surgery .
	manualset3
184122	4	414217	7	NULL	NULL	0	NULL	cardiac surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines postulated mechanisms for cerebral injury from cardiac surgery .
	manualset3
184123	1	414218	7	NULL	NULL	0	NULL	 article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines how a group of older women and men from a rural New York community deal with issues of meaning and purpose in their mature years , and compares their experiences with those of elders from India .
	manualset3
184124	2	414218	7	NULL	NULL	0	NULL	group 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines how a group of older women and men from a rural New York community deal with issues of meaning and purpose in their mature years , and compares their experiences with those of elders from India .
	manualset3
184125	3	414218	7	NULL	NULL	0	NULL	older women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines how a group of older women and men from a rural New York community deal with issues of meaning and purpose in their mature years , and compares their experiences with those of elders from India .
	manualset3
184127	4	414218	7	NULL	NULL	0	NULL	older men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines how a group of older women and men from a rural New York community deal with issues of meaning and purpose in their mature years , and compares their experiences with those of elders from India .
	manualset3
184128	5	414218	7	NULL	NULL	0	NULL	rural New York community	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines how a group of older women and men from a rural New York community deal with issues of meaning and purpose in their mature years , and compares their experiences with those of elders from India .
	manualset3
184129	6	414218	7	NULL	NULL	0	NULL	issues	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines how a group of older women and men from a rural New York community deal with issues of meaning and purpose in their mature years , and compares their experiences with those of elders from India .
	manualset3
184130	7	414218	7	NULL	NULL	0	NULL	mature years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines how a group of older women and men from a rural New York community deal with issues of meaning and purpose in their mature years , and compares their experiences with those of elders from India .
	manualset3
184131	8	414218	7	NULL	NULL	0	NULL	elders	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines how a group of older women and men from a rural New York community deal with issues of meaning and purpose in their mature years , and compares their experiences with those of elders from India .
	manualset3
184132	9	414218	7	NULL	NULL	0	NULL	 India	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines how a group of older women and men from a rural New York community deal with issues of meaning and purpose in their mature years , and compares their experiences with those of elders from India .
	manualset3
185705	10	414218	7	NULL	NULL	0	NULL	experiences	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines how a group of older women and men from a rural New York community deal with issues of meaning and purpose in their mature years , and compares their experiences with those of elders from India .
	manualset3
186236	11	414218	7	NULL	NULL	0	NULL	meaning	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines how a group of older women and men from a rural New York community deal with issues of meaning and purpose in their mature years , and compares their experiences with those of elders from India .
	manualset3
186237	12	414218	7	NULL	NULL	NULL	NULL	purpose	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This article examines how a group of older women and men from a rural New York community deal with issues of meaning and purpose in their mature years , and compares their experiences with those of elders from India .
	manualset3
184133	1	414219	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines the activities of two prominent migr scholars , Drs. Georg Leibbrandt ( 1899-1982 ) and Karl Stumpp ( 1896-1982 ) .
	manualset3
184134	2	414219	7	NULL	NULL	0	NULL	activities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines the activities of two prominent migr scholars , Drs. Georg Leibbrandt ( 1899-1982 ) and Karl Stumpp ( 1896-1982 ) .
	manualset3
184135	3	414219	7	NULL	NULL	NULL	NULL	prominent migr scholars	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This article examines the activities of two prominent migr scholars , Drs. Georg Leibbrandt ( 1899-1982 ) and Karl Stumpp ( 1896-1982 ) .
	manualset3
184136	4	414219	7	NULL	NULL	0	NULL	Drs. Georg Leibbrandt	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines the activities of two prominent migr scholars , Drs. Georg Leibbrandt ( 1899-1982 ) and Karl Stumpp ( 1896-1982 ) .
	manualset3
184137	5	414219	7	NULL	NULL	0	NULL	1899-1982	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines the activities of two prominent migr scholars , Drs. Georg Leibbrandt ( 1899-1982 ) and Karl Stumpp ( 1896-1982 ) .
	manualset3
184138	6	414219	7	NULL	NULL	0	NULL	Karl Stumpp	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines the activities of two prominent migr scholars , Drs. Georg Leibbrandt ( 1899-1982 ) and Karl Stumpp ( 1896-1982 ) .
	manualset3
184139	7	414219	7	NULL	NULL	0	NULL	1896-1982 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines the activities of two prominent migr scholars , Drs. Georg Leibbrandt ( 1899-1982 ) and Karl Stumpp ( 1896-1982 ) .
	manualset3
185706	8	414219	7	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines the activities of two prominent migr scholars , Drs. Georg Leibbrandt ( 1899-1982 ) and Karl Stumpp ( 1896-1982 ) .
	manualset3
184140	1	414220	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines the potential advantages and disadvantages of using silver in the management of chronic and burn wounds , and provides a physiological understanding of the body 's response to silver absorption .
	manualset3
184141	2	414220	7	NULL	NULL	NULL	NULL	 advantages	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This article examines the potential advantages and disadvantages of using silver in the management of chronic and burn wounds , and provides a physiological understanding of the body 's response to silver absorption .
	manualset3
184142	3	414220	7	NULL	NULL	0	NULL	disadvantages	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines the potential advantages and disadvantages of using silver in the management of chronic and burn wounds , and provides a physiological understanding of the body 's response to silver absorption .
	manualset3
184143	4	414220	7	NULL	NULL	0	NULL	silver	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines the potential advantages and disadvantages of using silver in the management of chronic and burn wounds , and provides a physiological understanding of the body 's response to silver absorption .
	manualset3
184144	5	414220	7	NULL	NULL	0	NULL	management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines the potential advantages and disadvantages of using silver in the management of chronic and burn wounds , and provides a physiological understanding of the body 's response to silver absorption .
	manualset3
184145	6	414220	7	NULL	NULL	0	NULL	chronic wounds	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines the potential advantages and disadvantages of using silver in the management of chronic and burn wounds , and provides a physiological understanding of the body 's response to silver absorption .
	manualset3
184146	7	414220	7	NULL	NULL	0	NULL	burn wounds	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines the potential advantages and disadvantages of using silver in the management of chronic and burn wounds , and provides a physiological understanding of the body 's response to silver absorption .
	manualset3
184147	8	414220	7	NULL	NULL	0	NULL	physiological understanding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines the potential advantages and disadvantages of using silver in the management of chronic and burn wounds , and provides a physiological understanding of the body 's response to silver absorption .
	manualset3
184148	9	414220	7	NULL	NULL	0	NULL	body 's response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines the potential advantages and disadvantages of using silver in the management of chronic and burn wounds , and provides a physiological understanding of the body 's response to silver absorption .
	manualset3
184149	10	414220	7	NULL	NULL	0	NULL	silver absorption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article examines the potential advantages and disadvantages of using silver in the management of chronic and burn wounds , and provides a physiological understanding of the body 's response to silver absorption .
	manualset3
184150	1	414221	7	NULL	NULL	0	NULL	 article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article explores why catheter fixation is important and some of the devices that can be used to achieve it .
	manualset3
184151	2	414221	7	NULL	NULL	0	NULL	catheter fixation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This article explores why catheter fixation is important and some of the devices that can be used to achieve it .
	manualset3
184152	3	414221	7	NULL	NULL	0	NULL	devices	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	This article explores why catheter fixation is important and some of the devices that can be used to achieve it .
	manualset3
184153	1	414222	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article gives an overview of the mechanisms of action of histone methyltransferases and demethylases , their role in the formation of certain diseases , and available inhibitors .
	manualset3
184154	2	414222	7	NULL	NULL	NULL	NULL	overview 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This article gives an overview of the mechanisms of action of histone methyltransferases and demethylases , their role in the formation of certain diseases , and available inhibitors .
	manualset3
184155	3	414222	7	NULL	NULL	NULL	NULL	mechanisms of action	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This article gives an overview of the mechanisms of action of histone methyltransferases and demethylases , their role in the formation of certain diseases , and available inhibitors .
	manualset3
184156	4	414222	7	NULL	NULL	0	NULL	histone methyltransferases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This article gives an overview of the mechanisms of action of histone methyltransferases and demethylases , their role in the formation of certain diseases , and available inhibitors .
	manualset3
184157	5	414222	7	NULL	NULL	0	NULL	demethylases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This article gives an overview of the mechanisms of action of histone methyltransferases and demethylases , their role in the formation of certain diseases , and available inhibitors .
	manualset3
184158	6	414222	7	NULL	NULL	0	NULL	 role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This article gives an overview of the mechanisms of action of histone methyltransferases and demethylases , their role in the formation of certain diseases , and available inhibitors .
	manualset3
184159	7	414222	7	NULL	NULL	0	NULL	formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This article gives an overview of the mechanisms of action of histone methyltransferases and demethylases , their role in the formation of certain diseases , and available inhibitors .
	manualset3
184160	8	414222	7	NULL	NULL	0	NULL	certain diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This article gives an overview of the mechanisms of action of histone methyltransferases and demethylases , their role in the formation of certain diseases , and available inhibitors .
	manualset3
184161	9	414222	7	NULL	NULL	0	NULL	inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This article gives an overview of the mechanisms of action of histone methyltransferases and demethylases , their role in the formation of certain diseases , and available inhibitors .
	manualset3
184221	1	414223	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article is an analytical review of current research addressing key factors of the home , the church , the community , and the healthcare system for creating partnerships to enhance community - based research in the African American community .
	manualset3
184222	2	414223	7	NULL	NULL	0	NULL	analytical review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article is an analytical review of current research addressing key factors of the home , the church , the community , and the healthcare system for creating partnerships to enhance community - based research in the African American community .
	manualset3
184223	3	414223	7	NULL	NULL	0	NULL	current research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article is an analytical review of current research addressing key factors of the home , the church , the community , and the healthcare system for creating partnerships to enhance community - based research in the African American community .
	manualset3
184227	4	414223	7	NULL	NULL	0	NULL	key factors	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	This article is an analytical review of current research addressing key factors of the home , the church , the community , and the healthcare system for creating partnerships to enhance community - based research in the African American community .
	manualset3
184229	5	414223	7	NULL	NULL	NULL	NULL	home	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This article is an analytical review of current research addressing key factors of the home , the church , the community , and the healthcare system for creating partnerships to enhance community - based research in the African American community .
	manualset3
184231	6	414223	7	NULL	NULL	0	NULL	church 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article is an analytical review of current research addressing key factors of the home , the church , the community , and the healthcare system for creating partnerships to enhance community - based research in the African American community .
	manualset3
184232	7	414223	7	NULL	NULL	0	NULL	community	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This article is an analytical review of current research addressing key factors of the home , the church , the community , and the healthcare system for creating partnerships to enhance community - based research in the African American community .
	manualset3
184234	8	414223	7	NULL	NULL	0	NULL	 healthcare system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	This article is an analytical review of current research addressing key factors of the home , the church , the community , and the healthcare system for creating partnerships to enhance community - based research in the African American community .
	manualset3
184235	9	414223	7	NULL	NULL	0	NULL	partnerships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	This article is an analytical review of current research addressing key factors of the home , the church , the community , and the healthcare system for creating partnerships to enhance community - based research in the African American community .
	manualset3
184236	10	414223	7	NULL	NULL	0	NULL	community - based research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article is an analytical review of current research addressing key factors of the home , the church , the community , and the healthcare system for creating partnerships to enhance community - based research in the African American community .
	manualset3
184237	11	414223	7	NULL	NULL	0	NULL	African American community	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This article is an analytical review of current research addressing key factors of the home , the church , the community , and the healthcare system for creating partnerships to enhance community - based research in the African American community .
	manualset3
184238	1	414224	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article is intended to provide an overview of the various methods used to study renal elimination of compounds .
	manualset3
184239	2	414224	7	NULL	NULL	0	NULL	 overview	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article is intended to provide an overview of the various methods used to study renal elimination of compounds .
	manualset3
184240	3	414224	7	NULL	NULL	0	NULL	methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article is intended to provide an overview of the various methods used to study renal elimination of compounds .
	manualset3
184241	4	414224	7	NULL	NULL	0	NULL	renal elimination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This article is intended to provide an overview of the various methods used to study renal elimination of compounds .
	manualset3
184242	5	414224	7	NULL	NULL	0	NULL	compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This article is intended to provide an overview of the various methods used to study renal elimination of compounds .
	manualset3
184243	1	414225	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article presents a hypothesis to explain the unequal diffusion of HIV among injection drug users in the United States by examining the distribution and use of one type of heroin -- `` Mexican black tar . ''
	manualset3
184245	2	414225	7	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This article presents a hypothesis to explain the unequal diffusion of HIV among injection drug users in the United States by examining the distribution and use of one type of heroin -- `` Mexican black tar . ''
	manualset3
184247	3	414225	7	NULL	NULL	0	NULL	unequal diffusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article presents a hypothesis to explain the unequal diffusion of HIV among injection drug users in the United States by examining the distribution and use of one type of heroin -- `` Mexican black tar . ''
	manualset3
184249	4	414225	7	NULL	NULL	0	NULL	HIV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	This article presents a hypothesis to explain the unequal diffusion of HIV among injection drug users in the United States by examining the distribution and use of one type of heroin -- `` Mexican black tar . ''
	manualset3
184251	5	414225	7	NULL	NULL	0	NULL	injection drug users	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This article presents a hypothesis to explain the unequal diffusion of HIV among injection drug users in the United States by examining the distribution and use of one type of heroin -- `` Mexican black tar . ''
	manualset3
184253	6	414225	7	NULL	NULL	0	NULL	United States	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article presents a hypothesis to explain the unequal diffusion of HIV among injection drug users in the United States by examining the distribution and use of one type of heroin -- `` Mexican black tar . ''
	manualset3
184254	7	414225	7	NULL	NULL	0	NULL	distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article presents a hypothesis to explain the unequal diffusion of HIV among injection drug users in the United States by examining the distribution and use of one type of heroin -- `` Mexican black tar . ''
	manualset3
184255	8	414225	7	NULL	NULL	0	NULL	one type	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article presents a hypothesis to explain the unequal diffusion of HIV among injection drug users in the United States by examining the distribution and use of one type of heroin -- `` Mexican black tar . ''
	manualset3
184257	9	414225	7	NULL	NULL	0	NULL	heroin -- `` Mexican black tar . ''	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	This article presents a hypothesis to explain the unequal diffusion of HIV among injection drug users in the United States by examining the distribution and use of one type of heroin -- `` Mexican black tar . ''
	manualset3
184271	1	414226	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article presents a review of literature on the current knowledge of IL-8 , its mechanisms of expression , and the effects it exerts on the neutrophil .
	manualset3
184272	2	414226	7	NULL	NULL	0	NULL	review of literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article presents a review of literature on the current knowledge of IL-8 , its mechanisms of expression , and the effects it exerts on the neutrophil .
	manualset3
184273	3	414226	7	NULL	NULL	0	NULL	knowledge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article presents a review of literature on the current knowledge of IL-8 , its mechanisms of expression , and the effects it exerts on the neutrophil .
	manualset3
184274	4	414226	7	NULL	NULL	0	NULL	 IL-8	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This article presents a review of literature on the current knowledge of IL-8 , its mechanisms of expression , and the effects it exerts on the neutrophil .
	manualset3
184275	5	414226	7	NULL	NULL	0	NULL	mechanisms 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This article presents a review of literature on the current knowledge of IL-8 , its mechanisms of expression , and the effects it exerts on the neutrophil .
	manualset3
184276	6	414226	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This article presents a review of literature on the current knowledge of IL-8 , its mechanisms of expression , and the effects it exerts on the neutrophil .
	manualset3
184277	7	414226	7	NULL	NULL	0	NULL	effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This article presents a review of literature on the current knowledge of IL-8 , its mechanisms of expression , and the effects it exerts on the neutrophil .
	manualset3
184278	8	414226	7	NULL	NULL	0	NULL	neutrophil	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	This article presents a review of literature on the current knowledge of IL-8 , its mechanisms of expression , and the effects it exerts on the neutrophil .
	manualset3
184279	1	414227	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article provides an overview of Medline-cited studies from 1980 to the present that examine the influence of ethnicity and socioeconomic status on the use of infertility services .
	manualset3
184280	2	414227	7	NULL	NULL	0	NULL	overview 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article provides an overview of Medline-cited studies from 1980 to the present that examine the influence of ethnicity and socioeconomic status on the use of infertility services .
	manualset3
184281	3	414227	7	NULL	NULL	0	NULL	Medline-cited studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article provides an overview of Medline-cited studies from 1980 to the present that examine the influence of ethnicity and socioeconomic status on the use of infertility services .
	manualset3
184282	4	414227	7	NULL	NULL	0	NULL	1980	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	This article provides an overview of Medline-cited studies from 1980 to the present that examine the influence of ethnicity and socioeconomic status on the use of infertility services .
	manualset3
184283	5	414227	7	NULL	NULL	0	NULL	influence of ethnicity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article provides an overview of Medline-cited studies from 1980 to the present that examine the influence of ethnicity and socioeconomic status on the use of infertility services .
	manualset3
184284	6	414227	7	NULL	NULL	0	NULL	socioeconomic status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article provides an overview of Medline-cited studies from 1980 to the present that examine the influence of ethnicity and socioeconomic status on the use of infertility services .
	manualset3
184285	7	414227	7	NULL	NULL	0	NULL	infertility services	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	This article provides an overview of Medline-cited studies from 1980 to the present that examine the influence of ethnicity and socioeconomic status on the use of infertility services .
	manualset3
184286	1	414228	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article provides an overview of the fundamental and inherent challenges in developing a health surveillance program for a health care facility .
	manualset3
184287	2	414228	7	NULL	NULL	0	NULL	overview	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article provides an overview of the fundamental and inherent challenges in developing a health surveillance program for a health care facility .
	manualset3
184288	3	414228	7	NULL	NULL	0	NULL	fundamental challenges	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article provides an overview of the fundamental and inherent challenges in developing a health surveillance program for a health care facility .
	manualset3
184289	4	414228	7	NULL	NULL	0	NULL	inherent challenges	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article provides an overview of the fundamental and inherent challenges in developing a health surveillance program for a health care facility .
	manualset3
184290	5	414228	7	NULL	NULL	0	NULL	developing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article provides an overview of the fundamental and inherent challenges in developing a health surveillance program for a health care facility .
	manualset3
184291	6	414228	7	NULL	NULL	0	NULL	health surveillance program	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	This article provides an overview of the fundamental and inherent challenges in developing a health surveillance program for a health care facility .
	manualset3
184292	7	414228	7	NULL	NULL	0	NULL	health care facility	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	This article provides an overview of the fundamental and inherent challenges in developing a health surveillance program for a health care facility .
	manualset3
184293	1	414229	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article provides an overview of the technique of magnetic resonance venography ( MRV ) and its relative value in the diagnostic work-up of suspected lower or upper extremity venous thrombosis .
	manualset3
184294	2	414229	7	NULL	NULL	0	NULL	overview 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article provides an overview of the technique of magnetic resonance venography ( MRV ) and its relative value in the diagnostic work-up of suspected lower or upper extremity venous thrombosis .
	manualset3
184295	3	414229	7	NULL	NULL	0	NULL	technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article provides an overview of the technique of magnetic resonance venography ( MRV ) and its relative value in the diagnostic work-up of suspected lower or upper extremity venous thrombosis .
	manualset3
184296	4	414229	7	NULL	NULL	0	NULL	magnetic resonance venography ( MRV )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article provides an overview of the technique of magnetic resonance venography ( MRV ) and its relative value in the diagnostic work-up of suspected lower or upper extremity venous thrombosis .
	manualset3
184297	5	414229	7	NULL	NULL	0	NULL	relative value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article provides an overview of the technique of magnetic resonance venography ( MRV ) and its relative value in the diagnostic work-up of suspected lower or upper extremity venous thrombosis .
	manualset3
184298	6	414229	7	NULL	NULL	0	NULL	diagnostic work-up	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This article provides an overview of the technique of magnetic resonance venography ( MRV ) and its relative value in the diagnostic work-up of suspected lower or upper extremity venous thrombosis .
	manualset3
184299	7	414229	7	NULL	NULL	0	NULL	suspected lower thrombosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article provides an overview of the technique of magnetic resonance venography ( MRV ) and its relative value in the diagnostic work-up of suspected lower or upper extremity venous thrombosis .
	manualset3
184300	8	414229	7	NULL	NULL	0	NULL	upper extremity venous thrombosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article provides an overview of the technique of magnetic resonance venography ( MRV ) and its relative value in the diagnostic work-up of suspected lower or upper extremity venous thrombosis .
	manualset3
184301	1	414230	7	NULL	NULL	0	NULL	article 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article relates the use of relative value units from its historical function of measuring productivity to how it has influenced the structure of national fee schedules .
	manualset3
184302	2	414230	7	NULL	NULL	0	NULL	relative value units	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article relates the use of relative value units from its historical function of measuring productivity to how it has influenced the structure of national fee schedules .
	manualset3
184303	3	414230	7	NULL	NULL	0	NULL	historical function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article relates the use of relative value units from its historical function of measuring productivity to how it has influenced the structure of national fee schedules .
	manualset3
184304	4	414230	7	NULL	NULL	0	NULL	measuring productivity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article relates the use of relative value units from its historical function of measuring productivity to how it has influenced the structure of national fee schedules .
	manualset3
184305	5	414230	7	NULL	NULL	0	NULL	structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article relates the use of relative value units from its historical function of measuring productivity to how it has influenced the structure of national fee schedules .
	manualset3
184306	6	414230	7	NULL	NULL	0	NULL	national fee schedules	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article relates the use of relative value units from its historical function of measuring productivity to how it has influenced the structure of national fee schedules .
	manualset3
184462	1	414231	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article represents an overview of the evaluation and diagnosis of stress urinary incontinence .
	manualset3
184463	2	414231	7	NULL	NULL	0	NULL	overview	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article represents an overview of the evaluation and diagnosis of stress urinary incontinence .
	manualset3
184464	3	414231	7	NULL	NULL	0	NULL	evaluation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This article represents an overview of the evaluation and diagnosis of stress urinary incontinence .
	manualset3
184465	4	414231	7	NULL	NULL	0	NULL	 diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article represents an overview of the evaluation and diagnosis of stress urinary incontinence .
	manualset3
184466	5	414231	7	NULL	NULL	0	NULL	stress urinary incontinence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article represents an overview of the evaluation and diagnosis of stress urinary incontinence .
	manualset3
184467	1	414232	7	NULL	NULL	0	NULL	Adenosine A1 receptor-mediated activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenosine A1 receptor-mediated activation of MAP kinase was abolished by pre-treatment with the protein tyrosine inhibitor , genistein ( 100 microM ; 6 + / -10 % of control ) .
	manualset3
184468	2	414232	7	NULL	NULL	0	NULL	MAP kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenosine A1 receptor-mediated activation of MAP kinase was abolished by pre-treatment with the protein tyrosine inhibitor , genistein ( 100 microM ; 6 + / -10 % of control ) .
	manualset3
184469	3	414232	7	NULL	NULL	0	NULL	pre-treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenosine A1 receptor-mediated activation of MAP kinase was abolished by pre-treatment with the protein tyrosine inhibitor , genistein ( 100 microM ; 6 + / -10 % of control ) .
	manualset3
184470	4	414232	7	NULL	NULL	0	NULL	protein tyrosine inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenosine A1 receptor-mediated activation of MAP kinase was abolished by pre-treatment with the protein tyrosine inhibitor , genistein ( 100 microM ; 6 + / -10 % of control ) .
	manualset3
184471	5	414232	7	NULL	NULL	0	NULL	genistein	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenosine A1 receptor-mediated activation of MAP kinase was abolished by pre-treatment with the protein tyrosine inhibitor , genistein ( 100 microM ; 6 + / -10 % of control ) .
	manualset3
184472	6	414232	7	NULL	NULL	0	NULL	100 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenosine A1 receptor-mediated activation of MAP kinase was abolished by pre-treatment with the protein tyrosine inhibitor , genistein ( 100 microM ; 6 + / -10 % of control ) .
	manualset3
184473	7	414232	7	NULL	NULL	0	NULL	6 + / -10 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenosine A1 receptor-mediated activation of MAP kinase was abolished by pre-treatment with the protein tyrosine inhibitor , genistein ( 100 microM ; 6 + / -10 % of control ) .
	manualset3
184474	8	414232	7	NULL	NULL	0	NULL	control	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenosine A1 receptor-mediated activation of MAP kinase was abolished by pre-treatment with the protein tyrosine inhibitor , genistein ( 100 microM ; 6 + / -10 % of control ) .
	manualset3
184475	1	414233	7	NULL	NULL	0	NULL	 article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews health and related research issues as well as to recommend improving interaction among community and all researchers .
	manualset3
184488	2	414233	7	NULL	NULL	0	NULL	health issues	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews health and related research issues as well as to recommend improving interaction among community and all researchers .
	manualset3
184489	3	414233	7	NULL	NULL	0	NULL	research issues	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews health and related research issues as well as to recommend improving interaction among community and all researchers .
	manualset3
184490	4	414233	7	NULL	NULL	NULL	NULL	interaction	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This article reviews health and related research issues as well as to recommend improving interaction among community and all researchers .
	manualset3
184491	5	414233	7	NULL	NULL	0	NULL	 community researchers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews health and related research issues as well as to recommend improving interaction among community and all researchers .
	manualset3
184492	6	414233	7	NULL	NULL	0	NULL	all researchers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews health and related research issues as well as to recommend improving interaction among community and all researchers .
	manualset3
184493	1	414234	7	NULL	NULL	0	NULL	 article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews recent discoveries in the area of antibiotics , premedication , genetics , obesity , tongue piercing , and tongue splitting .
	manualset3
184494	2	414234	7	NULL	NULL	0	NULL	discoveries	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews recent discoveries in the area of antibiotics , premedication , genetics , obesity , tongue piercing , and tongue splitting .
	manualset3
184495	3	414234	7	NULL	NULL	0	NULL	antibiotics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews recent discoveries in the area of antibiotics , premedication , genetics , obesity , tongue piercing , and tongue splitting .
	manualset3
184496	4	414234	7	NULL	NULL	0	NULL	premedication	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews recent discoveries in the area of antibiotics , premedication , genetics , obesity , tongue piercing , and tongue splitting .
	manualset3
184497	5	414234	7	NULL	NULL	0	NULL	genetics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews recent discoveries in the area of antibiotics , premedication , genetics , obesity , tongue piercing , and tongue splitting .
	manualset3
184498	6	414234	7	NULL	NULL	0	NULL	obesity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews recent discoveries in the area of antibiotics , premedication , genetics , obesity , tongue piercing , and tongue splitting .
	manualset3
184499	7	414234	7	NULL	NULL	0	NULL	tongue piercing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews recent discoveries in the area of antibiotics , premedication , genetics , obesity , tongue piercing , and tongue splitting .
	manualset3
184500	8	414234	7	NULL	NULL	0	NULL	tongue splitting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews recent discoveries in the area of antibiotics , premedication , genetics , obesity , tongue piercing , and tongue splitting .
	manualset3
184501	1	414235	7	NULL	NULL	0	NULL	article 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews recent research on drug abuse and addiction in Hispanics in which biological questions have been addressed , including work on genes , gene products ( proteins ) , physiology and pharmacotherapy .
	manualset3
184502	2	414235	7	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews recent research on drug abuse and addiction in Hispanics in which biological questions have been addressed , including work on genes , gene products ( proteins ) , physiology and pharmacotherapy .
	manualset3
184503	3	414235	7	NULL	NULL	0	NULL	drug abuse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews recent research on drug abuse and addiction in Hispanics in which biological questions have been addressed , including work on genes , gene products ( proteins ) , physiology and pharmacotherapy .
	manualset3
184504	4	414235	7	NULL	NULL	0	NULL	addiction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews recent research on drug abuse and addiction in Hispanics in which biological questions have been addressed , including work on genes , gene products ( proteins ) , physiology and pharmacotherapy .
	manualset3
184505	5	414235	7	NULL	NULL	0	NULL	Hispanics	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews recent research on drug abuse and addiction in Hispanics in which biological questions have been addressed , including work on genes , gene products ( proteins ) , physiology and pharmacotherapy .
	manualset3
184506	6	414235	7	NULL	NULL	0	NULL	biological questions	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews recent research on drug abuse and addiction in Hispanics in which biological questions have been addressed , including work on genes , gene products ( proteins ) , physiology and pharmacotherapy .
	manualset3
184507	7	414235	7	NULL	NULL	0	NULL	work	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews recent research on drug abuse and addiction in Hispanics in which biological questions have been addressed , including work on genes , gene products ( proteins ) , physiology and pharmacotherapy .
	manualset3
184508	8	414235	7	NULL	NULL	0	NULL	genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews recent research on drug abuse and addiction in Hispanics in which biological questions have been addressed , including work on genes , gene products ( proteins ) , physiology and pharmacotherapy .
	manualset3
184509	9	414235	7	NULL	NULL	0	NULL	gene products ( proteins )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews recent research on drug abuse and addiction in Hispanics in which biological questions have been addressed , including work on genes , gene products ( proteins ) , physiology and pharmacotherapy .
	manualset3
184510	10	414235	7	NULL	NULL	0	NULL	physiology 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews recent research on drug abuse and addiction in Hispanics in which biological questions have been addressed , including work on genes , gene products ( proteins ) , physiology and pharmacotherapy .
	manualset3
184511	11	414235	7	NULL	NULL	0	NULL	pharmacotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews recent research on drug abuse and addiction in Hispanics in which biological questions have been addressed , including work on genes , gene products ( proteins ) , physiology and pharmacotherapy .
	manualset3
184512	1	414236	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the applications of fMR imaging for studying the sensorimotor cortex prior to craniotomy .
	manualset3
184513	2	414236	7	NULL	NULL	0	NULL	applications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the applications of fMR imaging for studying the sensorimotor cortex prior to craniotomy .
	manualset3
184514	3	414236	7	NULL	NULL	0	NULL	fMR imaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the applications of fMR imaging for studying the sensorimotor cortex prior to craniotomy .
	manualset3
184515	4	414236	7	NULL	NULL	0	NULL	studying	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the applications of fMR imaging for studying the sensorimotor cortex prior to craniotomy .
	manualset3
184516	5	414236	7	NULL	NULL	0	NULL	sensorimotor cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the applications of fMR imaging for studying the sensorimotor cortex prior to craniotomy .
	manualset3
184517	6	414236	7	NULL	NULL	0	NULL	craniotomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the applications of fMR imaging for studying the sensorimotor cortex prior to craniotomy .
	manualset3
184518	1	414237	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the common and potentially serious thoracic sequelae in terms of pleural disease , pulmonary nodules , airways disorders , and interstitial disease , as well as pulmonary side effects of antirheumatic medication .
	manualset3
184519	2	414237	7	NULL	NULL	0	NULL	serious thoracic sequelae	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the common and potentially serious thoracic sequelae in terms of pleural disease , pulmonary nodules , airways disorders , and interstitial disease , as well as pulmonary side effects of antirheumatic medication .
	manualset3
184520	3	414237	7	NULL	NULL	0	NULL	pleural disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the common and potentially serious thoracic sequelae in terms of pleural disease , pulmonary nodules , airways disorders , and interstitial disease , as well as pulmonary side effects of antirheumatic medication .
	manualset3
184521	4	414237	7	NULL	NULL	0	NULL	pulmonary nodules	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the common and potentially serious thoracic sequelae in terms of pleural disease , pulmonary nodules , airways disorders , and interstitial disease , as well as pulmonary side effects of antirheumatic medication .
	manualset3
184522	5	414237	7	NULL	NULL	0	NULL	airways disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the common and potentially serious thoracic sequelae in terms of pleural disease , pulmonary nodules , airways disorders , and interstitial disease , as well as pulmonary side effects of antirheumatic medication .
	manualset3
184523	6	414237	7	NULL	NULL	0	NULL	interstitial disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the common and potentially serious thoracic sequelae in terms of pleural disease , pulmonary nodules , airways disorders , and interstitial disease , as well as pulmonary side effects of antirheumatic medication .
	manualset3
184524	7	414237	7	NULL	NULL	0	NULL	pulmonary side effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the common and potentially serious thoracic sequelae in terms of pleural disease , pulmonary nodules , airways disorders , and interstitial disease , as well as pulmonary side effects of antirheumatic medication .
	manualset3
184525	8	414237	7	NULL	NULL	0	NULL	antirheumatic medication	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the common and potentially serious thoracic sequelae in terms of pleural disease , pulmonary nodules , airways disorders , and interstitial disease , as well as pulmonary side effects of antirheumatic medication .
	manualset3
184526	1	414238	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the definition , measurement , associations , and putative mechanisms of selected positive psychological constructs on subjective and objective indicators of health with a focus on the latter half of the lifespan .
	manualset3
184527	2	414238	7	NULL	NULL	0	NULL	definition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the definition , measurement , associations , and putative mechanisms of selected positive psychological constructs on subjective and objective indicators of health with a focus on the latter half of the lifespan .
	manualset3
184528	3	414238	7	NULL	NULL	0	NULL	measurement	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the definition , measurement , associations , and putative mechanisms of selected positive psychological constructs on subjective and objective indicators of health with a focus on the latter half of the lifespan .
	manualset3
184529	4	414238	7	NULL	NULL	0	NULL	associations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the definition , measurement , associations , and putative mechanisms of selected positive psychological constructs on subjective and objective indicators of health with a focus on the latter half of the lifespan .
	manualset3
184530	5	414238	7	NULL	NULL	NULL	NULL	putative mechanisms	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This article reviews the definition , measurement , associations , and putative mechanisms of selected positive psychological constructs on subjective and objective indicators of health with a focus on the latter half of the lifespan .
	manualset3
184531	6	414238	7	NULL	NULL	0	NULL	selected positive psychological constructs	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the definition , measurement , associations , and putative mechanisms of selected positive psychological constructs on subjective and objective indicators of health with a focus on the latter half of the lifespan .
	manualset3
184532	7	414238	7	NULL	NULL	0	NULL	subjective indicators	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the definition , measurement , associations , and putative mechanisms of selected positive psychological constructs on subjective and objective indicators of health with a focus on the latter half of the lifespan .
	manualset3
184533	8	414238	7	NULL	NULL	0	NULL	objective indicators	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the definition , measurement , associations , and putative mechanisms of selected positive psychological constructs on subjective and objective indicators of health with a focus on the latter half of the lifespan .
	manualset3
184534	9	414238	7	NULL	NULL	0	NULL	health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the definition , measurement , associations , and putative mechanisms of selected positive psychological constructs on subjective and objective indicators of health with a focus on the latter half of the lifespan .
	manualset3
184535	10	414238	7	NULL	NULL	0	NULL	 latter half	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the definition , measurement , associations , and putative mechanisms of selected positive psychological constructs on subjective and objective indicators of health with a focus on the latter half of the lifespan .
	manualset3
184536	11	414238	7	NULL	NULL	0	NULL	 lifespan	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the definition , measurement , associations , and putative mechanisms of selected positive psychological constructs on subjective and objective indicators of health with a focus on the latter half of the lifespan .
	manualset3
184537	1	414239	7	NULL	NULL	0	NULL	article 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the epidemiologic evidence supporting an association between AD and two major vascular risk factors-blood pressure and diabetes .
	manualset3
184538	2	414239	7	NULL	NULL	0	NULL	epidemiologic evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the epidemiologic evidence supporting an association between AD and two major vascular risk factors-blood pressure and diabetes .
	manualset3
184539	3	414239	7	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the epidemiologic evidence supporting an association between AD and two major vascular risk factors-blood pressure and diabetes .
	manualset3
184540	4	414239	7	NULL	NULL	0	NULL	AD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the epidemiologic evidence supporting an association between AD and two major vascular risk factors-blood pressure and diabetes .
	manualset3
184541	5	414239	7	NULL	NULL	0	NULL	two major vascular risk factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the epidemiologic evidence supporting an association between AD and two major vascular risk factors-blood pressure and diabetes .
	manualset3
184542	6	414239	7	NULL	NULL	0	NULL	blood pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the epidemiologic evidence supporting an association between AD and two major vascular risk factors-blood pressure and diabetes .
	manualset3
184543	7	414239	7	NULL	NULL	0	NULL	diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the epidemiologic evidence supporting an association between AD and two major vascular risk factors-blood pressure and diabetes .
	manualset3
184544	1	414240	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the lesions commonly seen in biopsy specimens of human immunodeficiency virus infection and acquired immunodeficiency disease syndrome , their characteristic histologic features , and their differential diagnosis .
	manualset3
184545	2	414240	7	NULL	NULL	0	NULL	 lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the lesions commonly seen in biopsy specimens of human immunodeficiency virus infection and acquired immunodeficiency disease syndrome , their characteristic histologic features , and their differential diagnosis .
	manualset3
184546	3	414240	7	NULL	NULL	0	NULL	biopsy specimens 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the lesions commonly seen in biopsy specimens of human immunodeficiency virus infection and acquired immunodeficiency disease syndrome , their characteristic histologic features , and their differential diagnosis .
	manualset3
184547	4	414240	7	NULL	NULL	NULL	NULL	human immunodeficiency virus infection	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This article reviews the lesions commonly seen in biopsy specimens of human immunodeficiency virus infection and acquired immunodeficiency disease syndrome , their characteristic histologic features , and their differential diagnosis .
	manualset3
184548	5	414240	7	NULL	NULL	0	NULL	acquired immunodeficiency disease syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the lesions commonly seen in biopsy specimens of human immunodeficiency virus infection and acquired immunodeficiency disease syndrome , their characteristic histologic features , and their differential diagnosis .
	manualset3
184549	6	414240	7	NULL	NULL	0	NULL	histologic features	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the lesions commonly seen in biopsy specimens of human immunodeficiency virus infection and acquired immunodeficiency disease syndrome , their characteristic histologic features , and their differential diagnosis .
	manualset3
184550	7	414240	7	NULL	NULL	0	NULL	differential diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews the lesions commonly seen in biopsy specimens of human immunodeficiency virus infection and acquired immunodeficiency disease syndrome , their characteristic histologic features , and their differential diagnosis .
	manualset3
184568	1	414241	7	NULL	NULL	0	NULL	Adenovirus-mediated hepatic depletion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenovirus-mediated hepatic depletion of PRMT5 decreased SHP methylation and reversed the suppression of metabolic genes by SHP .
	manualset3
184569	2	414241	7	NULL	NULL	0	NULL	PRMT5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenovirus-mediated hepatic depletion of PRMT5 decreased SHP methylation and reversed the suppression of metabolic genes by SHP .
	manualset3
184571	3	414241	7	NULL	NULL	0	NULL	SHP methylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenovirus-mediated hepatic depletion of PRMT5 decreased SHP methylation and reversed the suppression of metabolic genes by SHP .
	manualset3
184575	4	414241	7	NULL	NULL	0	NULL	suppression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenovirus-mediated hepatic depletion of PRMT5 decreased SHP methylation and reversed the suppression of metabolic genes by SHP .
	manualset3
184576	5	414241	7	NULL	NULL	0	NULL	metabolic genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenovirus-mediated hepatic depletion of PRMT5 decreased SHP methylation and reversed the suppression of metabolic genes by SHP .
	manualset3
184577	6	414241	7	NULL	NULL	0	NULL	SHP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenovirus-mediated hepatic depletion of PRMT5 decreased SHP methylation and reversed the suppression of metabolic genes by SHP .
	manualset3
184578	1	414242	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article seeks to elucidate the trajectory of development in adolescents and adults with autism .
	manualset3
184579	2	414242	7	NULL	NULL	0	NULL	trajectory 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This article seeks to elucidate the trajectory of development in adolescents and adults with autism .
	manualset3
184580	3	414242	7	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This article seeks to elucidate the trajectory of development in adolescents and adults with autism .
	manualset3
184581	4	414242	7	NULL	NULL	0	NULL	adolescents 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This article seeks to elucidate the trajectory of development in adolescents and adults with autism .
	manualset3
184582	5	414242	7	NULL	NULL	0	NULL	adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This article seeks to elucidate the trajectory of development in adolescents and adults with autism .
	manualset3
184583	6	414242	7	NULL	NULL	0	NULL	autism	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This article seeks to elucidate the trajectory of development in adolescents and adults with autism .
	manualset3
184584	1	414243	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article seeks to provide an overview of common foot problems that are not related to diabetes mellitus .
	manualset3
184585	2	414243	7	NULL	NULL	0	NULL	overview 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article seeks to provide an overview of common foot problems that are not related to diabetes mellitus .
	manualset3
184586	3	414243	7	NULL	NULL	0	NULL	common foot problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article seeks to provide an overview of common foot problems that are not related to diabetes mellitus .
	manualset3
184587	4	414243	7	NULL	NULL	0	NULL	diabetes mellitus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This article seeks to provide an overview of common foot problems that are not related to diabetes mellitus .
	manualset3
184588	1	414244	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article will describe the Elder Abuse Resource Centre 's Peer Support Volunteer Program , beginning with the rationale for establishing this vital volunteer position .
	manualset3
184589	2	414244	7	NULL	NULL	0	NULL	Elder Abuse Resource Centre 's Peer Support Volunteer Program	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	This article will describe the Elder Abuse Resource Centre 's Peer Support Volunteer Program , beginning with the rationale for establishing this vital volunteer position .
	manualset3
184590	3	414244	7	NULL	NULL	0	NULL	rationale	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article will describe the Elder Abuse Resource Centre 's Peer Support Volunteer Program , beginning with the rationale for establishing this vital volunteer position .
	manualset3
184591	4	414244	7	NULL	NULL	0	NULL	volunteer position	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article will describe the Elder Abuse Resource Centre 's Peer Support Volunteer Program , beginning with the rationale for establishing this vital volunteer position .
	manualset3
184592	1	414245	7	NULL	NULL	0	NULL	 article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article will examine recent studies of synaptic transmission and plasticity in the amygdala in an effort to understand the relationships of these processes to aversive learning and memory .
	manualset3
184593	2	414245	7	NULL	NULL	0	NULL	recent studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article will examine recent studies of synaptic transmission and plasticity in the amygdala in an effort to understand the relationships of these processes to aversive learning and memory .
	manualset3
184594	3	414245	7	NULL	NULL	0	NULL	synaptic transmission	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This article will examine recent studies of synaptic transmission and plasticity in the amygdala in an effort to understand the relationships of these processes to aversive learning and memory .
	manualset3
184595	4	414245	7	NULL	NULL	0	NULL	plasticity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This article will examine recent studies of synaptic transmission and plasticity in the amygdala in an effort to understand the relationships of these processes to aversive learning and memory .
	manualset3
184596	5	414245	7	NULL	NULL	0	NULL	amygdala	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This article will examine recent studies of synaptic transmission and plasticity in the amygdala in an effort to understand the relationships of these processes to aversive learning and memory .
	manualset3
184597	6	414245	7	NULL	NULL	0	NULL	relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	This article will examine recent studies of synaptic transmission and plasticity in the amygdala in an effort to understand the relationships of these processes to aversive learning and memory .
	manualset3
184598	7	414245	7	NULL	NULL	0	NULL	processes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article will examine recent studies of synaptic transmission and plasticity in the amygdala in an effort to understand the relationships of these processes to aversive learning and memory .
	manualset3
184599	8	414245	7	NULL	NULL	0	NULL	learning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This article will examine recent studies of synaptic transmission and plasticity in the amygdala in an effort to understand the relationships of these processes to aversive learning and memory .
	manualset3
184600	9	414245	7	NULL	NULL	0	NULL	memory 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This article will examine recent studies of synaptic transmission and plasticity in the amygdala in an effort to understand the relationships of these processes to aversive learning and memory .
	manualset3
184601	1	414246	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article will first review why projects fail , then highlight the project management process used by McInnes Steel to specify , choose , and implement MRP II software that was `` right '' for them .
	manualset3
184602	2	414246	7	NULL	NULL	0	NULL	review	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article will first review why projects fail , then highlight the project management process used by McInnes Steel to specify , choose , and implement MRP II software that was `` right '' for them .
	manualset3
184603	3	414246	7	NULL	NULL	0	NULL	project management process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article will first review why projects fail , then highlight the project management process used by McInnes Steel to specify , choose , and implement MRP II software that was `` right '' for them .
	manualset3
184604	4	414246	7	NULL	NULL	0	NULL	McInnes Steel	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	This article will first review why projects fail , then highlight the project management process used by McInnes Steel to specify , choose , and implement MRP II software that was `` right '' for them .
	manualset3
184605	5	414246	7	NULL	NULL	0	NULL	MRP II software	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This article will first review why projects fail , then highlight the project management process used by McInnes Steel to specify , choose , and implement MRP II software that was `` right '' for them .
	manualset3
184606	6	414246	7	NULL	NULL	0	NULL	projects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article will first review why projects fail , then highlight the project management process used by McInnes Steel to specify , choose , and implement MRP II software that was `` right '' for them .
	manualset3
184607	1	414247	7	NULL	NULL	0	NULL	 assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This assay is an improvement on previously available colorimetric methods and could be easily incorporated into kits based on either an enzyme calibrant or the molar absorptivity of the phenol .
	manualset3
184608	2	414247	7	NULL	NULL	0	NULL	improvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This assay is an improvement on previously available colorimetric methods and could be easily incorporated into kits based on either an enzyme calibrant or the molar absorptivity of the phenol .
	manualset3
184609	3	414247	7	NULL	NULL	0	NULL	colorimetric methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This assay is an improvement on previously available colorimetric methods and could be easily incorporated into kits based on either an enzyme calibrant or the molar absorptivity of the phenol .
	manualset3
184610	4	414247	7	NULL	NULL	0	NULL	kits	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This assay is an improvement on previously available colorimetric methods and could be easily incorporated into kits based on either an enzyme calibrant or the molar absorptivity of the phenol .
	manualset3
184611	5	414247	7	NULL	NULL	0	NULL	enzyme calibrant	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This assay is an improvement on previously available colorimetric methods and could be easily incorporated into kits based on either an enzyme calibrant or the molar absorptivity of the phenol .
	manualset3
184612	6	414247	7	NULL	NULL	0	NULL	molar absorptivity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This assay is an improvement on previously available colorimetric methods and could be easily incorporated into kits based on either an enzyme calibrant or the molar absorptivity of the phenol .
	manualset3
184613	7	414247	7	NULL	NULL	0	NULL	phenol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This assay is an improvement on previously available colorimetric methods and could be easily incorporated into kits based on either an enzyme calibrant or the molar absorptivity of the phenol .
	manualset3
184614	1	414248	7	NULL	NULL	0	NULL	Adenylate cyclase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenylate cyclase activity in mononuclear leucocytes from patients with atopic dermatitis .
	manualset3
184615	2	414248	7	NULL	NULL	0	NULL	mononuclear leucocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenylate cyclase activity in mononuclear leucocytes from patients with atopic dermatitis .
	manualset3
184616	3	414248	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenylate cyclase activity in mononuclear leucocytes from patients with atopic dermatitis .
	manualset3
184617	4	414248	7	NULL	NULL	0	NULL	atopic dermatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenylate cyclase activity in mononuclear leucocytes from patients with atopic dermatitis .
	manualset3
184618	1	414249	7	NULL	NULL	0	NULL	bacterium	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	This bacterium significantly increased the fresh and dry weights of tomato seedlings grown in the presence of up to 172 mM NaCl salt .
	manualset3
184619	2	414249	7	NULL	NULL	0	NULL	 fresh weights	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This bacterium significantly increased the fresh and dry weights of tomato seedlings grown in the presence of up to 172 mM NaCl salt .
	manualset3
184620	3	414249	7	NULL	NULL	0	NULL	dry weights	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This bacterium significantly increased the fresh and dry weights of tomato seedlings grown in the presence of up to 172 mM NaCl salt .
	manualset3
184621	4	414249	7	NULL	NULL	0	NULL	tomato seedlings	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	This bacterium significantly increased the fresh and dry weights of tomato seedlings grown in the presence of up to 172 mM NaCl salt .
	manualset3
184622	5	414249	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This bacterium significantly increased the fresh and dry weights of tomato seedlings grown in the presence of up to 172 mM NaCl salt .
	manualset3
184623	6	414249	7	NULL	NULL	0	NULL	172 mM 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	This bacterium significantly increased the fresh and dry weights of tomato seedlings grown in the presence of up to 172 mM NaCl salt .
	manualset3
184624	7	414249	7	NULL	NULL	0	NULL	NaCl salt	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This bacterium significantly increased the fresh and dry weights of tomato seedlings grown in the presence of up to 172 mM NaCl salt .
	manualset3
184625	1	414250	7	NULL	NULL	0	NULL	 battery	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	This battery represents the Ah receptor ( AHR ) - mediated control of at least six , and probably many more , dioxin-inducible genes ; two cytochrome P450 genes-P450 1A1 and 1A2 ( Cypla1 , Cypla2-and four non-P450 genes , have experimentally been documented to be members of this battery .
	manualset3
184626	2	414250	7	NULL	NULL	0	NULL	Ah receptor ( AHR ) - mediated control	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This battery represents the Ah receptor ( AHR ) - mediated control of at least six , and probably many more , dioxin-inducible genes ; two cytochrome P450 genes-P450 1A1 and 1A2 ( Cypla1 , Cypla2-and four non-P450 genes , have experimentally been documented to be members of this battery .
	manualset3
184627	3	414250	7	NULL	NULL	0	NULL	six	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This battery represents the Ah receptor ( AHR ) - mediated control of at least six , and probably many more , dioxin-inducible genes ; two cytochrome P450 genes-P450 1A1 and 1A2 ( Cypla1 , Cypla2-and four non-P450 genes , have experimentally been documented to be members of this battery .
	manualset3
184628	4	414250	7	NULL	NULL	NULL	NULL	dioxin-inducible genes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This battery represents the Ah receptor ( AHR ) - mediated control of at least six , and probably many more , dioxin-inducible genes ; two cytochrome P450 genes-P450 1A1 and 1A2 ( Cypla1 , Cypla2-and four non-P450 genes , have experimentally been documented to be members of this battery .
	manualset3
184629	5	414250	7	NULL	NULL	0	NULL	 two cytochrome P450 genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This battery represents the Ah receptor ( AHR ) - mediated control of at least six , and probably many more , dioxin-inducible genes ; two cytochrome P450 genes-P450 1A1 and 1A2 ( Cypla1 , Cypla2-and four non-P450 genes , have experimentally been documented to be members of this battery .
	manualset3
184630	6	414250	7	NULL	NULL	0	NULL	P450 1A1 and 1A2 ( Cypla1 , Cypla2-	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This battery represents the Ah receptor ( AHR ) - mediated control of at least six , and probably many more , dioxin-inducible genes ; two cytochrome P450 genes-P450 1A1 and 1A2 ( Cypla1 , Cypla2-and four non-P450 genes , have experimentally been documented to be members of this battery .
	manualset3
184631	7	414250	7	NULL	NULL	0	NULL	four non-P450 genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This battery represents the Ah receptor ( AHR ) - mediated control of at least six , and probably many more , dioxin-inducible genes ; two cytochrome P450 genes-P450 1A1 and 1A2 ( Cypla1 , Cypla2-and four non-P450 genes , have experimentally been documented to be members of this battery .
	manualset3
184632	8	414250	7	NULL	NULL	0	NULL	 members	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This battery represents the Ah receptor ( AHR ) - mediated control of at least six , and probably many more , dioxin-inducible genes ; two cytochrome P450 genes-P450 1A1 and 1A2 ( Cypla1 , Cypla2-and four non-P450 genes , have experimentally been documented to be members of this battery .
	manualset3
184633	9	414250	7	NULL	NULL	0	NULL	battery	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	This battery represents the Ah receptor ( AHR ) - mediated control of at least six , and probably many more , dioxin-inducible genes ; two cytochrome P450 genes-P450 1A1 and 1A2 ( Cypla1 , Cypla2-and four non-P450 genes , have experimentally been documented to be members of this battery .
	manualset3
184634	1	414251	7	NULL	NULL	0	NULL	behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This behavior can be interpreted in terms of cell thickness fluctuations caused by thermally excited membrane undulations provided the range of wavelengths is small .
	manualset3
184635	2	414251	7	NULL	NULL	0	NULL	terms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This behavior can be interpreted in terms of cell thickness fluctuations caused by thermally excited membrane undulations provided the range of wavelengths is small .
	manualset3
184636	3	414251	7	NULL	NULL	0	NULL	cell thickness fluctuations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This behavior can be interpreted in terms of cell thickness fluctuations caused by thermally excited membrane undulations provided the range of wavelengths is small .
	manualset3
184637	4	414251	7	NULL	NULL	0	NULL	thermally excited membrane undulations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This behavior can be interpreted in terms of cell thickness fluctuations caused by thermally excited membrane undulations provided the range of wavelengths is small .
	manualset3
184638	5	414251	7	NULL	NULL	0	NULL	 range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This behavior can be interpreted in terms of cell thickness fluctuations caused by thermally excited membrane undulations provided the range of wavelengths is small .
	manualset3
184639	6	414251	7	NULL	NULL	0	NULL	wavelengths	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This behavior can be interpreted in terms of cell thickness fluctuations caused by thermally excited membrane undulations provided the range of wavelengths is small .
	manualset3
184640	1	414252	7	NULL	NULL	0	NULL	blinding patriotism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This blinding patriotism of even modest British people all over the world , gave the City , as well as the British Empire , a remarkable place in the world trade .
	manualset3
184641	2	414252	7	NULL	NULL	0	NULL	modest British people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This blinding patriotism of even modest British people all over the world , gave the City , as well as the British Empire , a remarkable place in the world trade .
	manualset3
184642	3	414252	7	NULL	NULL	0	NULL	world	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	This blinding patriotism of even modest British people all over the world , gave the City , as well as the British Empire , a remarkable place in the world trade .
	manualset3
184643	4	414252	7	NULL	NULL	0	NULL	City	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	This blinding patriotism of even modest British people all over the world , gave the City , as well as the British Empire , a remarkable place in the world trade .
	manualset3
184644	5	414252	7	NULL	NULL	0	NULL	British Empire	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	This blinding patriotism of even modest British people all over the world , gave the City , as well as the British Empire , a remarkable place in the world trade .
	manualset3
184645	6	414252	7	NULL	NULL	0	NULL	place	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	This blinding patriotism of even modest British people all over the world , gave the City , as well as the British Empire , a remarkable place in the world trade .
	manualset3
184646	7	414252	7	NULL	NULL	0	NULL	world trade	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This blinding patriotism of even modest British people all over the world , gave the City , as well as the British Empire , a remarkable place in the world trade .
	manualset3
184647	1	414253	7	NULL	NULL	0	NULL	booklet	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This booklet is Facts for Life , but more than a publication , it is a movement and the handbook of a grand alliance of communicators .
	manualset3
184648	2	414253	7	NULL	NULL	NULL	NULL	Facts for Life 	PublicationOrCitation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This booklet is Facts for Life , but more than a publication , it is a movement and the handbook of a grand alliance of communicators .
	manualset3
184649	3	414253	7	NULL	NULL	0	NULL	publication	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This booklet is Facts for Life , but more than a publication , it is a movement and the handbook of a grand alliance of communicators .
	manualset3
184650	4	414253	7	NULL	NULL	0	NULL	movement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This booklet is Facts for Life , but more than a publication , it is a movement and the handbook of a grand alliance of communicators .
	manualset3
184651	5	414253	7	NULL	NULL	0	NULL	handbook	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This booklet is Facts for Life , but more than a publication , it is a movement and the handbook of a grand alliance of communicators .
	manualset3
184652	6	414253	7	NULL	NULL	0	NULL	 grand alliance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This booklet is Facts for Life , but more than a publication , it is a movement and the handbook of a grand alliance of communicators .
	manualset3
184653	7	414253	7	NULL	NULL	0	NULL	communicators	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This booklet is Facts for Life , but more than a publication , it is a movement and the handbook of a grand alliance of communicators .
	manualset3
184654	1	414254	7	NULL	NULL	0	NULL	burden	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This burden , combined with the growing evidence for primary prevention from randomized controlled trials of structured lifestyle programs leads to recommendations to include caloric reduction , increased physical activity and specific assistance to patients in problem solving to achieve modest weight loss as well as pharmacotherapy .
	manualset3
184655	2	414254	7	NULL	NULL	0	NULL	growing evidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This burden , combined with the growing evidence for primary prevention from randomized controlled trials of structured lifestyle programs leads to recommendations to include caloric reduction , increased physical activity and specific assistance to patients in problem solving to achieve modest weight loss as well as pharmacotherapy .
	manualset3
184656	3	414254	7	NULL	NULL	0	NULL	primary prevention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This burden , combined with the growing evidence for primary prevention from randomized controlled trials of structured lifestyle programs leads to recommendations to include caloric reduction , increased physical activity and specific assistance to patients in problem solving to achieve modest weight loss as well as pharmacotherapy .
	manualset3
184657	4	414254	7	NULL	NULL	0	NULL	randomized controlled trials	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This burden , combined with the growing evidence for primary prevention from randomized controlled trials of structured lifestyle programs leads to recommendations to include caloric reduction , increased physical activity and specific assistance to patients in problem solving to achieve modest weight loss as well as pharmacotherapy .
	manualset3
184658	5	414254	7	NULL	NULL	0	NULL	structured lifestyle programs	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This burden , combined with the growing evidence for primary prevention from randomized controlled trials of structured lifestyle programs leads to recommendations to include caloric reduction , increased physical activity and specific assistance to patients in problem solving to achieve modest weight loss as well as pharmacotherapy .
	manualset3
184659	6	414254	7	NULL	NULL	0	NULL	recommendations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This burden , combined with the growing evidence for primary prevention from randomized controlled trials of structured lifestyle programs leads to recommendations to include caloric reduction , increased physical activity and specific assistance to patients in problem solving to achieve modest weight loss as well as pharmacotherapy .
	manualset3
184660	7	414254	7	NULL	NULL	0	NULL	caloric reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This burden , combined with the growing evidence for primary prevention from randomized controlled trials of structured lifestyle programs leads to recommendations to include caloric reduction , increased physical activity and specific assistance to patients in problem solving to achieve modest weight loss as well as pharmacotherapy .
	manualset3
184661	8	414254	7	NULL	NULL	0	NULL	 increased physical activity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This burden , combined with the growing evidence for primary prevention from randomized controlled trials of structured lifestyle programs leads to recommendations to include caloric reduction , increased physical activity and specific assistance to patients in problem solving to achieve modest weight loss as well as pharmacotherapy .
	manualset3
184662	9	414254	7	NULL	NULL	0	NULL	 specific assistance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This burden , combined with the growing evidence for primary prevention from randomized controlled trials of structured lifestyle programs leads to recommendations to include caloric reduction , increased physical activity and specific assistance to patients in problem solving to achieve modest weight loss as well as pharmacotherapy .
	manualset3
184663	10	414254	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This burden , combined with the growing evidence for primary prevention from randomized controlled trials of structured lifestyle programs leads to recommendations to include caloric reduction , increased physical activity and specific assistance to patients in problem solving to achieve modest weight loss as well as pharmacotherapy .
	manualset3
184664	11	414254	7	NULL	NULL	0	NULL	problem solving	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This burden , combined with the growing evidence for primary prevention from randomized controlled trials of structured lifestyle programs leads to recommendations to include caloric reduction , increased physical activity and specific assistance to patients in problem solving to achieve modest weight loss as well as pharmacotherapy .
	manualset3
184665	12	414254	7	NULL	NULL	0	NULL	modest weight loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This burden , combined with the growing evidence for primary prevention from randomized controlled trials of structured lifestyle programs leads to recommendations to include caloric reduction , increased physical activity and specific assistance to patients in problem solving to achieve modest weight loss as well as pharmacotherapy .
	manualset3
184666	13	414254	7	NULL	NULL	0	NULL	pharmacotherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This burden , combined with the growing evidence for primary prevention from randomized controlled trials of structured lifestyle programs leads to recommendations to include caloric reduction , increased physical activity and specific assistance to patients in problem solving to achieve modest weight loss as well as pharmacotherapy .
	manualset3
184667	1	414255	7	NULL	NULL	0	NULL	collagen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This can be defined again through the collagen .
	manualset3
184668	1	414256	7	NULL	NULL	0	NULL	in situ hybridization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This can be observed by in situ hybridization of tissue sections of 14.5-day-old mouse embryos , as well as by Northern blot analyses .
	manualset3
184669	2	414256	7	NULL	NULL	0	NULL	tissue sections	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	This can be observed by in situ hybridization of tissue sections of 14.5-day-old mouse embryos , as well as by Northern blot analyses .
	manualset3
184670	3	414256	7	NULL	NULL	0	NULL	14.5-day-old mouse embryos	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	This can be observed by in situ hybridization of tissue sections of 14.5-day-old mouse embryos , as well as by Northern blot analyses .
	manualset3
184671	4	414256	7	NULL	NULL	0	NULL	Northern blot analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This can be observed by in situ hybridization of tissue sections of 14.5-day-old mouse embryos , as well as by Northern blot analyses .
	manualset3
184672	1	414257	7	NULL	NULL	0	NULL	cardioprotection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This cardioprotection requires adenosine A ( 1 ) receptor signaling at the time of ischemia .
	manualset3
184673	2	414257	7	NULL	NULL	0	NULL	adenosine A ( 1 ) receptor signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This cardioprotection requires adenosine A ( 1 ) receptor signaling at the time of ischemia .
	manualset3
184674	3	414257	7	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	This cardioprotection requires adenosine A ( 1 ) receptor signaling at the time of ischemia .
	manualset3
184675	4	414257	7	NULL	NULL	0	NULL	ischemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This cardioprotection requires adenosine A ( 1 ) receptor signaling at the time of ischemia .
	manualset3
184676	1	414258	7	NULL	NULL	NULL	NULL	case	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This case clearly emphasizes the need for intensive monitoring of A-T patients for early signs of malignancy and the opportunity to consider specific and modified regimens of chemotherapy .
	manualset3
184677	2	414258	7	NULL	NULL	0	NULL	intensive monitoring	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This case clearly emphasizes the need for intensive monitoring of A-T patients for early signs of malignancy and the opportunity to consider specific and modified regimens of chemotherapy .
	manualset3
184678	3	414258	7	NULL	NULL	0	NULL	A-T patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This case clearly emphasizes the need for intensive monitoring of A-T patients for early signs of malignancy and the opportunity to consider specific and modified regimens of chemotherapy .
	manualset3
184679	4	414258	7	NULL	NULL	0	NULL	early signs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This case clearly emphasizes the need for intensive monitoring of A-T patients for early signs of malignancy and the opportunity to consider specific and modified regimens of chemotherapy .
	manualset3
184680	5	414258	7	NULL	NULL	0	NULL	malignancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This case clearly emphasizes the need for intensive monitoring of A-T patients for early signs of malignancy and the opportunity to consider specific and modified regimens of chemotherapy .
	manualset3
184681	6	414258	7	NULL	NULL	0	NULL	opportunity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This case clearly emphasizes the need for intensive monitoring of A-T patients for early signs of malignancy and the opportunity to consider specific and modified regimens of chemotherapy .
	manualset3
184682	7	414258	7	NULL	NULL	0	NULL	regimens	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This case clearly emphasizes the need for intensive monitoring of A-T patients for early signs of malignancy and the opportunity to consider specific and modified regimens of chemotherapy .
	manualset3
184683	8	414258	7	NULL	NULL	0	NULL	chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This case clearly emphasizes the need for intensive monitoring of A-T patients for early signs of malignancy and the opportunity to consider specific and modified regimens of chemotherapy .
	manualset3
184684	1	414259	7	NULL	NULL	0	NULL	case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This case demonstrates that right ventricular function can be restored following circulatory support with a mechanical assist device .
	manualset3
184685	2	414259	7	NULL	NULL	0	NULL	right ventricular function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This case demonstrates that right ventricular function can be restored following circulatory support with a mechanical assist device .
	manualset3
184686	3	414259	7	NULL	NULL	0	NULL	circulatory support	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This case demonstrates that right ventricular function can be restored following circulatory support with a mechanical assist device .
	manualset3
184687	4	414259	7	NULL	NULL	0	NULL	 mechanical assist device	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	This case demonstrates that right ventricular function can be restored following circulatory support with a mechanical assist device .
	manualset3
184688	1	414260	7	NULL	NULL	0	NULL	case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This case illustrates the complex reconstructive challenges of repairing an orbit in the setting of fistulization of the orbit with the maxillary sinus cavity .
	manualset3
184689	2	414260	7	NULL	NULL	0	NULL	complex reconstructive challenges	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This case illustrates the complex reconstructive challenges of repairing an orbit in the setting of fistulization of the orbit with the maxillary sinus cavity .
	manualset3
184690	3	414260	7	NULL	NULL	0	NULL	repairing an orbit	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This case illustrates the complex reconstructive challenges of repairing an orbit in the setting of fistulization of the orbit with the maxillary sinus cavity .
	manualset3
184691	4	414260	7	NULL	NULL	0	NULL	setting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This case illustrates the complex reconstructive challenges of repairing an orbit in the setting of fistulization of the orbit with the maxillary sinus cavity .
	manualset3
184692	5	414260	7	NULL	NULL	0	NULL	fistulization of the orbit	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This case illustrates the complex reconstructive challenges of repairing an orbit in the setting of fistulization of the orbit with the maxillary sinus cavity .
	manualset3
184693	6	414260	7	NULL	NULL	0	NULL	maxillary sinus cavity	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This case illustrates the complex reconstructive challenges of repairing an orbit in the setting of fistulization of the orbit with the maxillary sinus cavity .
	manualset3
184871	1	414261	7	NULL	NULL	0	NULL	case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This case is noteworthy for the finding of isolated lymphocyte predominant Hodgkin 's disease in the chest , the association of elevated serum 1 , 25-dihydroxyvitamin D with hypercalcemia that resolved postoperatively , and the uptake of thallium by the tumor .
	manualset3
184872	2	414261	7	NULL	NULL	0	NULL	 finding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This case is noteworthy for the finding of isolated lymphocyte predominant Hodgkin 's disease in the chest , the association of elevated serum 1 , 25-dihydroxyvitamin D with hypercalcemia that resolved postoperatively , and the uptake of thallium by the tumor .
	manualset3
184873	3	414261	7	NULL	NULL	0	NULL	 isolated lymphocyte	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	This case is noteworthy for the finding of isolated lymphocyte predominant Hodgkin 's disease in the chest , the association of elevated serum 1 , 25-dihydroxyvitamin D with hypercalcemia that resolved postoperatively , and the uptake of thallium by the tumor .
	manualset3
184874	4	414261	7	NULL	NULL	0	NULL	Hodgkin 's disease in the chest 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This case is noteworthy for the finding of isolated lymphocyte predominant Hodgkin 's disease in the chest , the association of elevated serum 1 , 25-dihydroxyvitamin D with hypercalcemia that resolved postoperatively , and the uptake of thallium by the tumor .
	manualset3
184875	5	414261	7	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	This case is noteworthy for the finding of isolated lymphocyte predominant Hodgkin 's disease in the chest , the association of elevated serum 1 , 25-dihydroxyvitamin D with hypercalcemia that resolved postoperatively , and the uptake of thallium by the tumor .
	manualset3
184876	6	414261	7	NULL	NULL	0	NULL	 serum 1 , 25-dihydroxyvitamin D	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This case is noteworthy for the finding of isolated lymphocyte predominant Hodgkin 's disease in the chest , the association of elevated serum 1 , 25-dihydroxyvitamin D with hypercalcemia that resolved postoperatively , and the uptake of thallium by the tumor .
	manualset3
184877	7	414261	7	NULL	NULL	0	NULL	hypercalcemia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This case is noteworthy for the finding of isolated lymphocyte predominant Hodgkin 's disease in the chest , the association of elevated serum 1 , 25-dihydroxyvitamin D with hypercalcemia that resolved postoperatively , and the uptake of thallium by the tumor .
	manualset3
184878	8	414261	7	NULL	NULL	0	NULL	uptake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This case is noteworthy for the finding of isolated lymphocyte predominant Hodgkin 's disease in the chest , the association of elevated serum 1 , 25-dihydroxyvitamin D with hypercalcemia that resolved postoperatively , and the uptake of thallium by the tumor .
	manualset3
184879	9	414261	7	NULL	NULL	0	NULL	thallium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This case is noteworthy for the finding of isolated lymphocyte predominant Hodgkin 's disease in the chest , the association of elevated serum 1 , 25-dihydroxyvitamin D with hypercalcemia that resolved postoperatively , and the uptake of thallium by the tumor .
	manualset3
184880	10	414261	7	NULL	NULL	0	NULL	 tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This case is noteworthy for the finding of isolated lymphocyte predominant Hodgkin 's disease in the chest , the association of elevated serum 1 , 25-dihydroxyvitamin D with hypercalcemia that resolved postoperatively , and the uptake of thallium by the tumor .
	manualset3
184881	1	414262	7	NULL	NULL	NULL	NULL	 case report	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This case report describes a successfully treated case of spontaneous rupture of bladder with ascites in a neonate with posterior urethral valves .
	manualset3
184883	3	414262	7	NULL	NULL	0	NULL	spontaneous rupture of bladder	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This case report describes a successfully treated case of spontaneous rupture of bladder with ascites in a neonate with posterior urethral valves .
	manualset3
184884	4	414262	7	NULL	NULL	0	NULL	ascites	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This case report describes a successfully treated case of spontaneous rupture of bladder with ascites in a neonate with posterior urethral valves .
	manualset3
184885	5	414262	7	NULL	NULL	0	NULL	neonate	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	This case report describes a successfully treated case of spontaneous rupture of bladder with ascites in a neonate with posterior urethral valves .
	manualset3
184886	6	414262	7	NULL	NULL	0	NULL	posterior urethral valves 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This case report describes a successfully treated case of spontaneous rupture of bladder with ascites in a neonate with posterior urethral valves .
	manualset3
184887	1	414263	7	NULL	NULL	0	NULL	Adequate staff amenities	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Adequate staff amenities and support space can foster increased staff satisfaction and thus lead to higher retention and recruitment rates .
	manualset3
184888	2	414263	7	NULL	NULL	0	NULL	support space 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Adequate staff amenities and support space can foster increased staff satisfaction and thus lead to higher retention and recruitment rates .
	manualset3
184889	3	414263	7	NULL	NULL	0	NULL	 increased staff satisfaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Adequate staff amenities and support space can foster increased staff satisfaction and thus lead to higher retention and recruitment rates .
	manualset3
184890	4	414263	7	NULL	NULL	0	NULL	higher retention rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Adequate staff amenities and support space can foster increased staff satisfaction and thus lead to higher retention and recruitment rates .
	manualset3
184891	5	414263	7	NULL	NULL	0	NULL	recruitment rates 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Adequate staff amenities and support space can foster increased staff satisfaction and thus lead to higher retention and recruitment rates .
	manualset3
184892	1	414264	7	NULL	NULL	0	NULL	case report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This case report documents a substantial increase in chest wall expansion in a middle-aged woman with stable right thoracic spinal curvature due to idiopathic scoliosis .
	manualset3
184893	2	414264	7	NULL	NULL	0	NULL	substantial increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This case report documents a substantial increase in chest wall expansion in a middle-aged woman with stable right thoracic spinal curvature due to idiopathic scoliosis .
	manualset3
184894	3	414264	7	NULL	NULL	0	NULL	 chest wall expansion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This case report documents a substantial increase in chest wall expansion in a middle-aged woman with stable right thoracic spinal curvature due to idiopathic scoliosis .
	manualset3
184895	4	414264	7	NULL	NULL	0	NULL	middle-aged woman	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	This case report documents a substantial increase in chest wall expansion in a middle-aged woman with stable right thoracic spinal curvature due to idiopathic scoliosis .
	manualset3
184896	5	414264	7	NULL	NULL	0	NULL	stable right thoracic spinal curvature	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This case report documents a substantial increase in chest wall expansion in a middle-aged woman with stable right thoracic spinal curvature due to idiopathic scoliosis .
	manualset3
184897	6	414264	7	NULL	NULL	0	NULL	idiopathic scoliosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This case report documents a substantial increase in chest wall expansion in a middle-aged woman with stable right thoracic spinal curvature due to idiopathic scoliosis .
	manualset3
184898	1	414265	7	NULL	NULL	NULL	NULL	 cell line	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This cell line , designated BLIN-1 , was initially established in tissue culture medium containing low m.w. B cell growth factor , and consistently shows a dependency on this cytokine for optimal growth at low density .
	manualset3
184899	2	414265	7	NULL	NULL	0	NULL	BLIN-1	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	This cell line , designated BLIN-1 , was initially established in tissue culture medium containing low m.w. B cell growth factor , and consistently shows a dependency on this cytokine for optimal growth at low density .
	manualset3
184900	3	414265	7	NULL	NULL	0	NULL	tissue culture medium 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	This cell line , designated BLIN-1 , was initially established in tissue culture medium containing low m.w. B cell growth factor , and consistently shows a dependency on this cytokine for optimal growth at low density .
	manualset3
184901	4	414265	7	NULL	NULL	0	NULL	low m.w.	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This cell line , designated BLIN-1 , was initially established in tissue culture medium containing low m.w. B cell growth factor , and consistently shows a dependency on this cytokine for optimal growth at low density .
	manualset3
184902	5	414265	7	NULL	NULL	NULL	NULL	B cell growth factor	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This cell line , designated BLIN-1 , was initially established in tissue culture medium containing low m.w. B cell growth factor , and consistently shows a dependency on this cytokine for optimal growth at low density .
	manualset3
184903	6	414265	7	NULL	NULL	0	NULL	cytokine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This cell line , designated BLIN-1 , was initially established in tissue culture medium containing low m.w. B cell growth factor , and consistently shows a dependency on this cytokine for optimal growth at low density .
	manualset3
184904	7	414265	7	NULL	NULL	0	NULL	optimal growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This cell line , designated BLIN-1 , was initially established in tissue culture medium containing low m.w. B cell growth factor , and consistently shows a dependency on this cytokine for optimal growth at low density .
	manualset3
184905	8	414265	7	NULL	NULL	0	NULL	low density	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This cell line , designated BLIN-1 , was initially established in tissue culture medium containing low m.w. B cell growth factor , and consistently shows a dependency on this cytokine for optimal growth at low density .
	manualset3
184906	1	414266	7	NULL	NULL	0	NULL	cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	This cell line expresses only slightly reduced levels of DNA-PKcs but has undetectable DNA-PK activity .
	manualset3
184907	2	414266	7	NULL	NULL	0	NULL	reduced levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This cell line expresses only slightly reduced levels of DNA-PKcs but has undetectable DNA-PK activity .
	manualset3
184908	3	414266	7	NULL	NULL	0	NULL	DNA-PKcs	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This cell line expresses only slightly reduced levels of DNA-PKcs but has undetectable DNA-PK activity .
	manualset3
184909	4	414266	7	NULL	NULL	0	NULL	DNA-PK activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This cell line expresses only slightly reduced levels of DNA-PKcs but has undetectable DNA-PK activity .
	manualset3
184910	1	414267	7	NULL	NULL	0	NULL	censoring	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This censoring may arise from a number of sources , one of which being the possibility that less severe crashes may be under-reported and thus may be less likely to appear in crash databases .
	manualset3
184911	2	414267	7	NULL	NULL	NULL	NULL	number of sources	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This censoring may arise from a number of sources , one of which being the possibility that less severe crashes may be under-reported and thus may be less likely to appear in crash databases .
	manualset3
184912	3	414267	7	NULL	NULL	0	NULL	one 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This censoring may arise from a number of sources , one of which being the possibility that less severe crashes may be under-reported and thus may be less likely to appear in crash databases .
	manualset3
184913	4	414267	7	NULL	NULL	0	NULL	less severe crashes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This censoring may arise from a number of sources , one of which being the possibility that less severe crashes may be under-reported and thus may be less likely to appear in crash databases .
	manualset3
184914	5	414267	7	NULL	NULL	0	NULL	crash databases	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This censoring may arise from a number of sources , one of which being the possibility that less severe crashes may be under-reported and thus may be less likely to appear in crash databases .
	manualset3
187537	6	414267	7	NULL	NULL	0	NULL	possibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This censoring may arise from a number of sources , one of which being the possibility that less severe crashes may be under-reported and thus may be less likely to appear in crash databases .
	manualset3
184915	1	414268	7	NULL	NULL	0	NULL	change	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This change was accompanied by increase in liver weights and centrilobular hepatocyte hypertrophy .
	manualset3
184916	2	414268	7	NULL	NULL	0	NULL	 increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This change was accompanied by increase in liver weights and centrilobular hepatocyte hypertrophy .
	manualset3
184917	3	414268	7	NULL	NULL	0	NULL	 liver weights	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This change was accompanied by increase in liver weights and centrilobular hepatocyte hypertrophy .
	manualset3
184918	4	414268	7	NULL	NULL	0	NULL	centrilobular hepatocyte hypertrophy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This change was accompanied by increase in liver weights and centrilobular hepatocyte hypertrophy .
	manualset3
184919	1	414269	7	NULL	NULL	0	NULL	cloned double-stranded PSTV cDNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	This cloned double-stranded PSTV cDNA contains the cleavage sites for six restriction endonucleases predicted by the published primary sequence of PSTV as well as one additional site each for Ava I , Hae III , Hpa II , and Sma I. The additional Ava I , Hpa II , and Sma I sites are explained by the presence of a second C-C-C-G-G-G sequence in the cloned double-stranded cDNA .
	manualset3
184920	2	414269	7	NULL	NULL	NULL	NULL	cleavage sites	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This cloned double-stranded PSTV cDNA contains the cleavage sites for six restriction endonucleases predicted by the published primary sequence of PSTV as well as one additional site each for Ava I , Hae III , Hpa II , and Sma I. The additional Ava I , Hpa II , and Sma I sites are explained by the presence of a second C-C-C-G-G-G sequence in the cloned double-stranded cDNA .
	manualset3
184921	3	414269	7	NULL	NULL	0	NULL	six restriction endonucleases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This cloned double-stranded PSTV cDNA contains the cleavage sites for six restriction endonucleases predicted by the published primary sequence of PSTV as well as one additional site each for Ava I , Hae III , Hpa II , and Sma I. The additional Ava I , Hpa II , and Sma I sites are explained by the presence of a second C-C-C-G-G-G sequence in the cloned double-stranded cDNA .
	manualset3
184922	4	414269	7	NULL	NULL	0	NULL	published primary sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	This cloned double-stranded PSTV cDNA contains the cleavage sites for six restriction endonucleases predicted by the published primary sequence of PSTV as well as one additional site each for Ava I , Hae III , Hpa II , and Sma I. The additional Ava I , Hpa II , and Sma I sites are explained by the presence of a second C-C-C-G-G-G sequence in the cloned double-stranded cDNA .
	manualset3
184923	5	414269	7	NULL	NULL	0	NULL	PSTV	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	This cloned double-stranded PSTV cDNA contains the cleavage sites for six restriction endonucleases predicted by the published primary sequence of PSTV as well as one additional site each for Ava I , Hae III , Hpa II , and Sma I. The additional Ava I , Hpa II , and Sma I sites are explained by the presence of a second C-C-C-G-G-G sequence in the cloned double-stranded cDNA .
	manualset3
184924	6	414269	7	NULL	NULL	NULL	NULL	one additional site 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This cloned double-stranded PSTV cDNA contains the cleavage sites for six restriction endonucleases predicted by the published primary sequence of PSTV as well as one additional site each for Ava I , Hae III , Hpa II , and Sma I. The additional Ava I , Hpa II , and Sma I sites are explained by the presence of a second C-C-C-G-G-G sequence in the cloned double-stranded cDNA .
	manualset3
184925	7	414269	7	NULL	NULL	0	NULL	 Ava I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This cloned double-stranded PSTV cDNA contains the cleavage sites for six restriction endonucleases predicted by the published primary sequence of PSTV as well as one additional site each for Ava I , Hae III , Hpa II , and Sma I. The additional Ava I , Hpa II , and Sma I sites are explained by the presence of a second C-C-C-G-G-G sequence in the cloned double-stranded cDNA .
	manualset3
184926	8	414269	7	NULL	NULL	0	NULL	Hae III	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This cloned double-stranded PSTV cDNA contains the cleavage sites for six restriction endonucleases predicted by the published primary sequence of PSTV as well as one additional site each for Ava I , Hae III , Hpa II , and Sma I. The additional Ava I , Hpa II , and Sma I sites are explained by the presence of a second C-C-C-G-G-G sequence in the cloned double-stranded cDNA .
	manualset3
184927	9	414269	7	NULL	NULL	0	NULL	Hpa II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This cloned double-stranded PSTV cDNA contains the cleavage sites for six restriction endonucleases predicted by the published primary sequence of PSTV as well as one additional site each for Ava I , Hae III , Hpa II , and Sma I. The additional Ava I , Hpa II , and Sma I sites are explained by the presence of a second C-C-C-G-G-G sequence in the cloned double-stranded cDNA .
	manualset3
184928	10	414269	7	NULL	NULL	0	NULL	Sma I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This cloned double-stranded PSTV cDNA contains the cleavage sites for six restriction endonucleases predicted by the published primary sequence of PSTV as well as one additional site each for Ava I , Hae III , Hpa II , and Sma I. The additional Ava I , Hpa II , and Sma I sites are explained by the presence of a second C-C-C-G-G-G sequence in the cloned double-stranded cDNA .
	manualset3
184929	11	414269	7	NULL	NULL	NULL	NULL	Ava I sites	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This cloned double-stranded PSTV cDNA contains the cleavage sites for six restriction endonucleases predicted by the published primary sequence of PSTV as well as one additional site each for Ava I , Hae III , Hpa II , and Sma I. The additional Ava I , Hpa II , and Sma I sites are explained by the presence of a second C-C-C-G-G-G sequence in the cloned double-stranded cDNA .
	manualset3
184930	12	414269	7	NULL	NULL	NULL	NULL	Hpa II sites	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This cloned double-stranded PSTV cDNA contains the cleavage sites for six restriction endonucleases predicted by the published primary sequence of PSTV as well as one additional site each for Ava I , Hae III , Hpa II , and Sma I. The additional Ava I , Hpa II , and Sma I sites are explained by the presence of a second C-C-C-G-G-G sequence in the cloned double-stranded cDNA .
	manualset3
184931	13	414269	7	NULL	NULL	0	NULL	Sma I sites 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	This cloned double-stranded PSTV cDNA contains the cleavage sites for six restriction endonucleases predicted by the published primary sequence of PSTV as well as one additional site each for Ava I , Hae III , Hpa II , and Sma I. The additional Ava I , Hpa II , and Sma I sites are explained by the presence of a second C-C-C-G-G-G sequence in the cloned double-stranded cDNA .
	manualset3
184932	14	414269	7	NULL	NULL	0	NULL	 presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This cloned double-stranded PSTV cDNA contains the cleavage sites for six restriction endonucleases predicted by the published primary sequence of PSTV as well as one additional site each for Ava I , Hae III , Hpa II , and Sma I. The additional Ava I , Hpa II , and Sma I sites are explained by the presence of a second C-C-C-G-G-G sequence in the cloned double-stranded cDNA .
	manualset3
184933	15	414269	7	NULL	NULL	0	NULL	second C-C-C-G-G-G sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	This cloned double-stranded PSTV cDNA contains the cleavage sites for six restriction endonucleases predicted by the published primary sequence of PSTV as well as one additional site each for Ava I , Hae III , Hpa II , and Sma I. The additional Ava I , Hpa II , and Sma I sites are explained by the presence of a second C-C-C-G-G-G sequence in the cloned double-stranded cDNA .
	manualset3
184934	16	414269	7	NULL	NULL	0	NULL	cloned double-stranded cDNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	This cloned double-stranded PSTV cDNA contains the cleavage sites for six restriction endonucleases predicted by the published primary sequence of PSTV as well as one additional site each for Ava I , Hae III , Hpa II , and Sma I. The additional Ava I , Hpa II , and Sma I sites are explained by the presence of a second C-C-C-G-G-G sequence in the cloned double-stranded cDNA .
	manualset3
184935	1	414270	7	NULL	NULL	NULL	NULL	 co-elution	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This co-elution of diacylglycerols with monohydroxy polyunsaturated fatty acids can lead to a significant error in estimation of lipoxygenation activity by conversion of radiolabeled precursors , because the incorporation of fatty acids into diacylglycerols is very active in many tissues .
	manualset3
184936	2	414270	7	NULL	NULL	0	NULL	diacylglycerols	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This co-elution of diacylglycerols with monohydroxy polyunsaturated fatty acids can lead to a significant error in estimation of lipoxygenation activity by conversion of radiolabeled precursors , because the incorporation of fatty acids into diacylglycerols is very active in many tissues .
	manualset3
184937	3	414270	7	NULL	NULL	0	NULL	monohydroxy polyunsaturated fatty acids 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This co-elution of diacylglycerols with monohydroxy polyunsaturated fatty acids can lead to a significant error in estimation of lipoxygenation activity by conversion of radiolabeled precursors , because the incorporation of fatty acids into diacylglycerols is very active in many tissues .
	manualset3
184938	4	414270	7	NULL	NULL	0	NULL	significant error 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This co-elution of diacylglycerols with monohydroxy polyunsaturated fatty acids can lead to a significant error in estimation of lipoxygenation activity by conversion of radiolabeled precursors , because the incorporation of fatty acids into diacylglycerols is very active in many tissues .
	manualset3
184939	5	414270	7	NULL	NULL	0	NULL	estimation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This co-elution of diacylglycerols with monohydroxy polyunsaturated fatty acids can lead to a significant error in estimation of lipoxygenation activity by conversion of radiolabeled precursors , because the incorporation of fatty acids into diacylglycerols is very active in many tissues .
	manualset3
184940	6	414270	7	NULL	NULL	0	NULL	 lipoxygenation activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This co-elution of diacylglycerols with monohydroxy polyunsaturated fatty acids can lead to a significant error in estimation of lipoxygenation activity by conversion of radiolabeled precursors , because the incorporation of fatty acids into diacylglycerols is very active in many tissues .
	manualset3
184941	7	414270	7	NULL	NULL	NULL	NULL	conversion	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This co-elution of diacylglycerols with monohydroxy polyunsaturated fatty acids can lead to a significant error in estimation of lipoxygenation activity by conversion of radiolabeled precursors , because the incorporation of fatty acids into diacylglycerols is very active in many tissues .
	manualset3
184942	8	414270	7	NULL	NULL	0	NULL	 radiolabeled precursors 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This co-elution of diacylglycerols with monohydroxy polyunsaturated fatty acids can lead to a significant error in estimation of lipoxygenation activity by conversion of radiolabeled precursors , because the incorporation of fatty acids into diacylglycerols is very active in many tissues .
	manualset3
184943	9	414270	7	NULL	NULL	0	NULL	incorporation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This co-elution of diacylglycerols with monohydroxy polyunsaturated fatty acids can lead to a significant error in estimation of lipoxygenation activity by conversion of radiolabeled precursors , because the incorporation of fatty acids into diacylglycerols is very active in many tissues .
	manualset3
184944	10	414270	7	NULL	NULL	0	NULL	fatty acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This co-elution of diacylglycerols with monohydroxy polyunsaturated fatty acids can lead to a significant error in estimation of lipoxygenation activity by conversion of radiolabeled precursors , because the incorporation of fatty acids into diacylglycerols is very active in many tissues .
	manualset3
184945	11	414270	7	NULL	NULL	0	NULL	diacylglycerols	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This co-elution of diacylglycerols with monohydroxy polyunsaturated fatty acids can lead to a significant error in estimation of lipoxygenation activity by conversion of radiolabeled precursors , because the incorporation of fatty acids into diacylglycerols is very active in many tissues .
	manualset3
184946	12	414270	7	NULL	NULL	0	NULL	tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	This co-elution of diacylglycerols with monohydroxy polyunsaturated fatty acids can lead to a significant error in estimation of lipoxygenation activity by conversion of radiolabeled precursors , because the incorporation of fatty acids into diacylglycerols is very active in many tissues .
	manualset3
184947	1	414271	7	NULL	NULL	0	NULL	Adherence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Adherence to evidence-based guidelines can have a profound and positive impact on patient outcomes and healthcare costs .
	manualset3
184948	2	414271	7	NULL	NULL	0	NULL	evidence-based guidelines	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Adherence to evidence-based guidelines can have a profound and positive impact on patient outcomes and healthcare costs .
	manualset3
184949	3	414271	7	NULL	NULL	0	NULL	 positive impact 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Adherence to evidence-based guidelines can have a profound and positive impact on patient outcomes and healthcare costs .
	manualset3
184950	4	414271	7	NULL	NULL	0	NULL	patient outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Adherence to evidence-based guidelines can have a profound and positive impact on patient outcomes and healthcare costs .
	manualset3
184951	5	414271	7	NULL	NULL	0	NULL	healthcare costs	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Adherence to evidence-based guidelines can have a profound and positive impact on patient outcomes and healthcare costs .
	manualset3
184952	1	414272	7	NULL	NULL	0	NULL	colony color phenotype	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	This colony color phenotype is very useful for genetic screens and may be applicable for use in other yeast species .
	manualset3
184953	2	414272	7	NULL	NULL	0	NULL	genetic screens	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This colony color phenotype is very useful for genetic screens and may be applicable for use in other yeast species .
	manualset3
184954	3	414272	7	NULL	NULL	0	NULL	 applicable	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This colony color phenotype is very useful for genetic screens and may be applicable for use in other yeast species .
	manualset3
184955	4	414272	7	NULL	NULL	0	NULL	yeast species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	This colony color phenotype is very useful for genetic screens and may be applicable for use in other yeast species .
	manualset3
184956	1	414273	7	NULL	NULL	0	NULL	complete transition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This complete transition was coupled to a sharp shortening of the OHO and NHO hydrogen bonds at & lt ; 100 K , the appearance of new additional positions of the protons in these H-bonds , and a slight strengthening of the C-HO bonds formed by methyl-groups .
	manualset3
184957	2	414273	7	NULL	NULL	0	NULL	sharp shortening	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This complete transition was coupled to a sharp shortening of the OHO and NHO hydrogen bonds at & lt ; 100 K , the appearance of new additional positions of the protons in these H-bonds , and a slight strengthening of the C-HO bonds formed by methyl-groups .
	manualset3
184958	3	414273	7	NULL	NULL	0	NULL	OHO hydrogen bond	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This complete transition was coupled to a sharp shortening of the OHO and NHO hydrogen bonds at & lt ; 100 K , the appearance of new additional positions of the protons in these H-bonds , and a slight strengthening of the C-HO bonds formed by methyl-groups .
	manualset3
184959	4	414273	7	NULL	NULL	0	NULL	NHO hydrogen bonds	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This complete transition was coupled to a sharp shortening of the OHO and NHO hydrogen bonds at & lt ; 100 K , the appearance of new additional positions of the protons in these H-bonds , and a slight strengthening of the C-HO bonds formed by methyl-groups .
	manualset3
184960	5	414273	7	NULL	NULL	0	NULL	& lt	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This complete transition was coupled to a sharp shortening of the OHO and NHO hydrogen bonds at & lt ; 100 K , the appearance of new additional positions of the protons in these H-bonds , and a slight strengthening of the C-HO bonds formed by methyl-groups .
	manualset3
184961	6	414273	7	NULL	NULL	0	NULL	100 K	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	This complete transition was coupled to a sharp shortening of the OHO and NHO hydrogen bonds at & lt ; 100 K , the appearance of new additional positions of the protons in these H-bonds , and a slight strengthening of the C-HO bonds formed by methyl-groups .
	manualset3
184962	7	414273	7	NULL	NULL	0	NULL	appearance	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This complete transition was coupled to a sharp shortening of the OHO and NHO hydrogen bonds at & lt ; 100 K , the appearance of new additional positions of the protons in these H-bonds , and a slight strengthening of the C-HO bonds formed by methyl-groups .
	manualset3
184963	8	414273	7	NULL	NULL	0	NULL	new additional positions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This complete transition was coupled to a sharp shortening of the OHO and NHO hydrogen bonds at & lt ; 100 K , the appearance of new additional positions of the protons in these H-bonds , and a slight strengthening of the C-HO bonds formed by methyl-groups .
	manualset3
184964	9	414273	7	NULL	NULL	0	NULL	protons	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	This complete transition was coupled to a sharp shortening of the OHO and NHO hydrogen bonds at & lt ; 100 K , the appearance of new additional positions of the protons in these H-bonds , and a slight strengthening of the C-HO bonds formed by methyl-groups .
	manualset3
184965	10	414273	7	NULL	NULL	0	NULL	H-bonds	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This complete transition was coupled to a sharp shortening of the OHO and NHO hydrogen bonds at & lt ; 100 K , the appearance of new additional positions of the protons in these H-bonds , and a slight strengthening of the C-HO bonds formed by methyl-groups .
	manualset3
184966	11	414273	7	NULL	NULL	0	NULL	strengthening	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This complete transition was coupled to a sharp shortening of the OHO and NHO hydrogen bonds at & lt ; 100 K , the appearance of new additional positions of the protons in these H-bonds , and a slight strengthening of the C-HO bonds formed by methyl-groups .
	manualset3
184967	12	414273	7	NULL	NULL	0	NULL	C-HO bonds	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This complete transition was coupled to a sharp shortening of the OHO and NHO hydrogen bonds at & lt ; 100 K , the appearance of new additional positions of the protons in these H-bonds , and a slight strengthening of the C-HO bonds formed by methyl-groups .
	manualset3
184968	13	414273	7	NULL	NULL	0	NULL	methyl-groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This complete transition was coupled to a sharp shortening of the OHO and NHO hydrogen bonds at & lt ; 100 K , the appearance of new additional positions of the protons in these H-bonds , and a slight strengthening of the C-HO bonds formed by methyl-groups .
	manualset3
184969	1	414274	7	NULL	NULL	0	NULL	complex	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	This complex displays a markedly upfield ( 195 ) Pt NMR shift compared to tetraphenylporphyrinatoplatinum ( II ) .
	manualset3
184970	2	414274	7	NULL	NULL	0	NULL	upfield ( 195 ) Pt NMR shift	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This complex displays a markedly upfield ( 195 ) Pt NMR shift compared to tetraphenylporphyrinatoplatinum ( II ) .
	manualset3
184971	3	414274	7	NULL	NULL	0	NULL	tetraphenylporphyrinatoplatinum ( II )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This complex displays a markedly upfield ( 195 ) Pt NMR shift compared to tetraphenylporphyrinatoplatinum ( II ) .
	manualset3
184972	1	414275	7	NULL	NULL	0	NULL	 compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This compound can suppress both serum and 24-hr urine estrogens to a greater extent than produced by the second generation inhibitor , CGS 16949A .
	manualset3
184973	2	414275	7	NULL	NULL	0	NULL	serum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This compound can suppress both serum and 24-hr urine estrogens to a greater extent than produced by the second generation inhibitor , CGS 16949A .
	manualset3
184974	3	414275	7	NULL	NULL	NULL	NULL	24-hr urine estrogens	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This compound can suppress both serum and 24-hr urine estrogens to a greater extent than produced by the second generation inhibitor , CGS 16949A .
	manualset3
184975	4	414275	7	NULL	NULL	0	NULL	second generation inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This compound can suppress both serum and 24-hr urine estrogens to a greater extent than produced by the second generation inhibitor , CGS 16949A .
	manualset3
184976	5	414275	7	NULL	NULL	0	NULL	CGS 16949A	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This compound can suppress both serum and 24-hr urine estrogens to a greater extent than produced by the second generation inhibitor , CGS 16949A .
	manualset3
184977	1	414276	7	NULL	NULL	0	NULL	compound	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	This compound was equally as efficient as linezolid in reducing the production of lesions .
	manualset3
184978	2	414276	7	NULL	NULL	0	NULL	linezolid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This compound was equally as efficient as linezolid in reducing the production of lesions .
	manualset3
184979	3	414276	7	NULL	NULL	0	NULL	production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This compound was equally as efficient as linezolid in reducing the production of lesions .
	manualset3
184980	4	414276	7	NULL	NULL	0	NULL	lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This compound was equally as efficient as linezolid in reducing the production of lesions .
	manualset3
184981	1	414277	7	NULL	NULL	0	NULL	concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This concentration killed 41 % of the Daudi cells and 42 % of the Ramos cells .
	manualset3
184982	2	414277	7	NULL	NULL	0	NULL	41 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	This concentration killed 41 % of the Daudi cells and 42 % of the Ramos cells .
	manualset3
184983	3	414277	7	NULL	NULL	0	NULL	Daudi cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	This concentration killed 41 % of the Daudi cells and 42 % of the Ramos cells .
	manualset3
184984	4	414277	7	NULL	NULL	0	NULL	42 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	This concentration killed 41 % of the Daudi cells and 42 % of the Ramos cells .
	manualset3
184985	5	414277	7	NULL	NULL	0	NULL	Ramos cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	This concentration killed 41 % of the Daudi cells and 42 % of the Ramos cells .
	manualset3
184986	1	414278	7	NULL	NULL	0	NULL	concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This concentration should be `` safe '' for D. magna under prevailing conditions ( reconstituted water with a hardness of 250 mg l-1 as CaCo3 and a synthetic diet based on fish food and baby gruel ) .
	manualset3
184987	2	414278	7	NULL	NULL	0	NULL	D. magna	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	This concentration should be `` safe '' for D. magna under prevailing conditions ( reconstituted water with a hardness of 250 mg l-1 as CaCo3 and a synthetic diet based on fish food and baby gruel ) .
	manualset3
184988	3	414278	7	NULL	NULL	0	NULL	prevailing conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	This concentration should be `` safe '' for D. magna under prevailing conditions ( reconstituted water with a hardness of 250 mg l-1 as CaCo3 and a synthetic diet based on fish food and baby gruel ) .
	manualset3
184989	4	414278	7	NULL	NULL	0	NULL	 reconstituted water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This concentration should be `` safe '' for D. magna under prevailing conditions ( reconstituted water with a hardness of 250 mg l-1 as CaCo3 and a synthetic diet based on fish food and baby gruel ) .
	manualset3
184990	5	414278	7	NULL	NULL	0	NULL	hardness	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This concentration should be `` safe '' for D. magna under prevailing conditions ( reconstituted water with a hardness of 250 mg l-1 as CaCo3 and a synthetic diet based on fish food and baby gruel ) .
	manualset3
184991	6	414278	7	NULL	NULL	0	NULL	250 mg l-1 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	This concentration should be `` safe '' for D. magna under prevailing conditions ( reconstituted water with a hardness of 250 mg l-1 as CaCo3 and a synthetic diet based on fish food and baby gruel ) .
	manualset3
184992	7	414278	7	NULL	NULL	0	NULL	CaCo3	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This concentration should be `` safe '' for D. magna under prevailing conditions ( reconstituted water with a hardness of 250 mg l-1 as CaCo3 and a synthetic diet based on fish food and baby gruel ) .
	manualset3
184993	8	414278	7	NULL	NULL	0	NULL	synthetic diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	This concentration should be `` safe '' for D. magna under prevailing conditions ( reconstituted water with a hardness of 250 mg l-1 as CaCo3 and a synthetic diet based on fish food and baby gruel ) .
	manualset3
184994	9	414278	7	NULL	NULL	0	NULL	 fish food 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	This concentration should be `` safe '' for D. magna under prevailing conditions ( reconstituted water with a hardness of 250 mg l-1 as CaCo3 and a synthetic diet based on fish food and baby gruel ) .
	manualset3
184995	10	414278	7	NULL	NULL	0	NULL	baby gruel 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	This concentration should be `` safe '' for D. magna under prevailing conditions ( reconstituted water with a hardness of 250 mg l-1 as CaCo3 and a synthetic diet based on fish food and baby gruel ) .
	manualset3
184996	1	414279	7	NULL	NULL	0	NULL	Adherence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Adherence to the Mediterranean diet was evaluated with the modified-MedDietScore ( theoretical range 0-75 ) , while assessment of the metabolic syndrome ( MetS ) was based on the third Adult Treatment Panel ( ( ATP III ) National Cholesterol Education Program ) criteria .
	manualset3
184997	2	414279	7	NULL	NULL	0	NULL	Mediterranean diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Adherence to the Mediterranean diet was evaluated with the modified-MedDietScore ( theoretical range 0-75 ) , while assessment of the metabolic syndrome ( MetS ) was based on the third Adult Treatment Panel ( ( ATP III ) National Cholesterol Education Program ) criteria .
	manualset3
184998	3	414279	7	NULL	NULL	0	NULL	modified-MedDietScore	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Adherence to the Mediterranean diet was evaluated with the modified-MedDietScore ( theoretical range 0-75 ) , while assessment of the metabolic syndrome ( MetS ) was based on the third Adult Treatment Panel ( ( ATP III ) National Cholesterol Education Program ) criteria .
	manualset3
184999	4	414279	7	NULL	NULL	0	NULL	theoretical range 0-75	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Adherence to the Mediterranean diet was evaluated with the modified-MedDietScore ( theoretical range 0-75 ) , while assessment of the metabolic syndrome ( MetS ) was based on the third Adult Treatment Panel ( ( ATP III ) National Cholesterol Education Program ) criteria .
	manualset3
185000	5	414279	7	NULL	NULL	0	NULL	assessment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Adherence to the Mediterranean diet was evaluated with the modified-MedDietScore ( theoretical range 0-75 ) , while assessment of the metabolic syndrome ( MetS ) was based on the third Adult Treatment Panel ( ( ATP III ) National Cholesterol Education Program ) criteria .
	manualset3
185001	6	414279	7	NULL	NULL	0	NULL	metabolic syndrome ( MetS )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Adherence to the Mediterranean diet was evaluated with the modified-MedDietScore ( theoretical range 0-75 ) , while assessment of the metabolic syndrome ( MetS ) was based on the third Adult Treatment Panel ( ( ATP III ) National Cholesterol Education Program ) criteria .
	manualset3
185002	7	414279	7	NULL	NULL	0	NULL	third Adult Treatment Panel ( ( ATP III ) National Cholesterol Education Program )	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Adherence to the Mediterranean diet was evaluated with the modified-MedDietScore ( theoretical range 0-75 ) , while assessment of the metabolic syndrome ( MetS ) was based on the third Adult Treatment Panel ( ( ATP III ) National Cholesterol Education Program ) criteria .
	manualset3
189772	8	414279	7	NULL	NULL	0	NULL	criteria	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Adherence to the Mediterranean diet was evaluated with the modified-MedDietScore ( theoretical range 0-75 ) , while assessment of the metabolic syndrome ( MetS ) was based on the third Adult Treatment Panel ( ( ATP III ) National Cholesterol Education Program ) criteria .
	manualset3
185003	1	414280	7	NULL	NULL	0	NULL	conception	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This conception of the relation between the subjective and the objective foreshadows his later , and controversial , concept of synchronicity , which is , Jung insists , a way of apprehending the world in terms of its meaning .
	manualset3
185004	2	414280	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	This conception of the relation between the subjective and the objective foreshadows his later , and controversial , concept of synchronicity , which is , Jung insists , a way of apprehending the world in terms of its meaning .
	manualset3
185005	3	414280	7	NULL	NULL	0	NULL	subjective foreshadows	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This conception of the relation between the subjective and the objective foreshadows his later , and controversial , concept of synchronicity , which is , Jung insists , a way of apprehending the world in terms of its meaning .
	manualset3
185006	4	414280	7	NULL	NULL	0	NULL	objective foreshadows	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This conception of the relation between the subjective and the objective foreshadows his later , and controversial , concept of synchronicity , which is , Jung insists , a way of apprehending the world in terms of its meaning .
	manualset3
185007	5	414280	7	NULL	NULL	0	NULL	concept of synchronicity	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This conception of the relation between the subjective and the objective foreshadows his later , and controversial , concept of synchronicity , which is , Jung insists , a way of apprehending the world in terms of its meaning .
	manualset3
185008	6	414280	7	NULL	NULL	0	NULL	Jung	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	This conception of the relation between the subjective and the objective foreshadows his later , and controversial , concept of synchronicity , which is , Jung insists , a way of apprehending the world in terms of its meaning .
	manualset3
185009	7	414280	7	NULL	NULL	0	NULL	way	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This conception of the relation between the subjective and the objective foreshadows his later , and controversial , concept of synchronicity , which is , Jung insists , a way of apprehending the world in terms of its meaning .
	manualset3
185010	8	414280	7	NULL	NULL	0	NULL	apprehending	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This conception of the relation between the subjective and the objective foreshadows his later , and controversial , concept of synchronicity , which is , Jung insists , a way of apprehending the world in terms of its meaning .
	manualset3
185011	9	414280	7	NULL	NULL	0	NULL	world	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	This conception of the relation between the subjective and the objective foreshadows his later , and controversial , concept of synchronicity , which is , Jung insists , a way of apprehending the world in terms of its meaning .
	manualset3
185012	10	414280	7	NULL	NULL	0	NULL	meaning 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This conception of the relation between the subjective and the objective foreshadows his later , and controversial , concept of synchronicity , which is , Jung insists , a way of apprehending the world in terms of its meaning .
	manualset3
185013	1	414281	7	NULL	NULL	0	NULL	conclusion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This conclusion is still valid after correcting for lipophilicity ( ClogP ) and molecular size , as well as any potential protein target bias in the data sets .
	manualset3
185014	2	414281	7	NULL	NULL	0	NULL	 lipophilicity ( ClogP )	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	This conclusion is still valid after correcting for lipophilicity ( ClogP ) and molecular size , as well as any potential protein target bias in the data sets .
	manualset3
185015	3	414281	7	NULL	NULL	0	NULL	molecular size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This conclusion is still valid after correcting for lipophilicity ( ClogP ) and molecular size , as well as any potential protein target bias in the data sets .
	manualset3
185016	4	414281	7	NULL	NULL	0	NULL	potential protein target bias	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This conclusion is still valid after correcting for lipophilicity ( ClogP ) and molecular size , as well as any potential protein target bias in the data sets .
	manualset3
185017	5	414281	7	NULL	NULL	0	NULL	data sets	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	This conclusion is still valid after correcting for lipophilicity ( ClogP ) and molecular size , as well as any potential protein target bias in the data sets .
	manualset3
185018	1	414282	7	NULL	NULL	0	NULL	conclusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This conclusion was consistent with the observation that treatment of immunopurified , affinity-labeled receptors with calf intestine alkaline phosphatase did not alter the apparent pI values or distribution of the steroid-binding protein isoforms .
	manualset3
185019	2	414282	7	NULL	NULL	0	NULL	observation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This conclusion was consistent with the observation that treatment of immunopurified , affinity-labeled receptors with calf intestine alkaline phosphatase did not alter the apparent pI values or distribution of the steroid-binding protein isoforms .
	manualset3
185020	3	414282	7	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This conclusion was consistent with the observation that treatment of immunopurified , affinity-labeled receptors with calf intestine alkaline phosphatase did not alter the apparent pI values or distribution of the steroid-binding protein isoforms .
	manualset3
185021	4	414282	7	NULL	NULL	0	NULL	immunopurified , affinity-labeled receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This conclusion was consistent with the observation that treatment of immunopurified , affinity-labeled receptors with calf intestine alkaline phosphatase did not alter the apparent pI values or distribution of the steroid-binding protein isoforms .
	manualset3
185022	5	414282	7	NULL	NULL	0	NULL	calf intestine alkaline phosphatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This conclusion was consistent with the observation that treatment of immunopurified , affinity-labeled receptors with calf intestine alkaline phosphatase did not alter the apparent pI values or distribution of the steroid-binding protein isoforms .
	manualset3
185023	6	414282	7	NULL	NULL	0	NULL	pI values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This conclusion was consistent with the observation that treatment of immunopurified , affinity-labeled receptors with calf intestine alkaline phosphatase did not alter the apparent pI values or distribution of the steroid-binding protein isoforms .
	manualset3
185024	7	414282	7	NULL	NULL	0	NULL	distribution 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This conclusion was consistent with the observation that treatment of immunopurified , affinity-labeled receptors with calf intestine alkaline phosphatase did not alter the apparent pI values or distribution of the steroid-binding protein isoforms .
	manualset3
185025	8	414282	7	NULL	NULL	NULL	NULL	steroid-binding protein isoforms 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This conclusion was consistent with the observation that treatment of immunopurified , affinity-labeled receptors with calf intestine alkaline phosphatase did not alter the apparent pI values or distribution of the steroid-binding protein isoforms .
	manualset3
185026	1	414283	7	NULL	NULL	0	NULL	condition	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	This condition will continue as the industry adjusts to government and marketplace pressures .
	manualset3
185027	2	414283	7	NULL	NULL	0	NULL	industry	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	This condition will continue as the industry adjusts to government and marketplace pressures .
	manualset3
185028	3	414283	7	NULL	NULL	0	NULL	government pressures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This condition will continue as the industry adjusts to government and marketplace pressures .
	manualset3
185029	4	414283	7	NULL	NULL	0	NULL	marketplace pressures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This condition will continue as the industry adjusts to government and marketplace pressures .
	manualset3
185030	1	414284	7	NULL	NULL	0	NULL	constantly growing database	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This constantly growing database has become a key resource in the field of DNA methylation research .
	manualset3
185031	2	414284	7	NULL	NULL	NULL	NULL	key resource	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This constantly growing database has become a key resource in the field of DNA methylation research .
	manualset3
185032	3	414284	7	NULL	NULL	0	NULL	 field	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This constantly growing database has become a key resource in the field of DNA methylation research .
	manualset3
185033	4	414284	7	NULL	NULL	0	NULL	DNA methylation research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This constantly growing database has become a key resource in the field of DNA methylation research .
	manualset3
185034	1	414285	7	NULL	NULL	0	NULL	continuing process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This continuing process results in the formation of contraction clumps in which the contractile filaments form an increasingly homogeneous mass. .
	manualset3
185035	2	414285	7	NULL	NULL	0	NULL	formation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This continuing process results in the formation of contraction clumps in which the contractile filaments form an increasingly homogeneous mass. .
	manualset3
185036	3	414285	7	NULL	NULL	0	NULL	contraction clumps	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This continuing process results in the formation of contraction clumps in which the contractile filaments form an increasingly homogeneous mass. .
	manualset3
185037	4	414285	7	NULL	NULL	0	NULL	contractile filaments	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This continuing process results in the formation of contraction clumps in which the contractile filaments form an increasingly homogeneous mass. .
	manualset3
185038	5	414285	7	NULL	NULL	0	NULL	increasingly homogeneous mass	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This continuing process results in the formation of contraction clumps in which the contractile filaments form an increasingly homogeneous mass. .
	manualset3
185039	1	414286	7	NULL	NULL	0	NULL	contrasts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This contrasts markedly to the situation in vivo , where uptake has been demonstrated in the majority of tumors investigated .
	manualset3
185040	2	414286	7	NULL	NULL	0	NULL	situation	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	This contrasts markedly to the situation in vivo , where uptake has been demonstrated in the majority of tumors investigated .
	manualset3
185041	3	414286	7	NULL	NULL	0	NULL	uptake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This contrasts markedly to the situation in vivo , where uptake has been demonstrated in the majority of tumors investigated .
	manualset3
185042	4	414286	7	NULL	NULL	0	NULL	tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This contrasts markedly to the situation in vivo , where uptake has been demonstrated in the majority of tumors investigated .
	manualset3
185043	1	414287	7	NULL	NULL	0	NULL	de novo expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This contrasts with the profound de novo expression of TLR2 following a single systemic injection of the lipopolysaccharide ( LPS ) .
	manualset3
185044	2	414287	7	NULL	NULL	0	NULL	TLR2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This contrasts with the profound de novo expression of TLR2 following a single systemic injection of the lipopolysaccharide ( LPS ) .
	manualset3
185045	3	414287	7	NULL	NULL	0	NULL	single systemic injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This contrasts with the profound de novo expression of TLR2 following a single systemic injection of the lipopolysaccharide ( LPS ) .
	manualset3
185046	4	414287	7	NULL	NULL	0	NULL	lipopolysaccharide ( LPS )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This contrasts with the profound de novo expression of TLR2 following a single systemic injection of the lipopolysaccharide ( LPS ) .
	manualset3
185047	1	414288	7	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	This correlation was even more evident for the patients who had clinically relevant relapses during the 30 months of follow-up ( seven of 11 patients ) .
	manualset3
185048	2	414288	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This correlation was even more evident for the patients who had clinically relevant relapses during the 30 months of follow-up ( seven of 11 patients ) .
	manualset3
185049	3	414288	7	NULL	NULL	0	NULL	relapses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This correlation was even more evident for the patients who had clinically relevant relapses during the 30 months of follow-up ( seven of 11 patients ) .
	manualset3
185050	4	414288	7	NULL	NULL	0	NULL	30 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	This correlation was even more evident for the patients who had clinically relevant relapses during the 30 months of follow-up ( seven of 11 patients ) .
	manualset3
185051	5	414288	7	NULL	NULL	0	NULL	follow-up	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This correlation was even more evident for the patients who had clinically relevant relapses during the 30 months of follow-up ( seven of 11 patients ) .
	manualset3
185052	6	414288	7	NULL	NULL	0	NULL	seven patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This correlation was even more evident for the patients who had clinically relevant relapses during the 30 months of follow-up ( seven of 11 patients ) .
	manualset3
185053	7	414288	7	NULL	NULL	0	NULL	11 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This correlation was even more evident for the patients who had clinically relevant relapses during the 30 months of follow-up ( seven of 11 patients ) .
	manualset3
185054	1	414289	7	NULL	NULL	0	NULL	DNA replication	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This could advance DNA replication and cleavage in the first cell cycle , resulting in increased cell numbers .
	manualset3
185055	2	414289	7	NULL	NULL	0	NULL	cleavage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This could advance DNA replication and cleavage in the first cell cycle , resulting in increased cell numbers .
	manualset3
185056	3	414289	7	NULL	NULL	NULL	NULL	first cell cycle	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This could advance DNA replication and cleavage in the first cell cycle , resulting in increased cell numbers .
	manualset3
185057	4	414289	7	NULL	NULL	0	NULL	cell numbers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This could advance DNA replication and cleavage in the first cell cycle , resulting in increased cell numbers .
	manualset3
185058	1	414290	7	NULL	NULL	0	NULL	effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This could be due to the effect of Mood Disorder on personality .
	manualset3
185059	2	414290	7	NULL	NULL	0	NULL	Mood Disorder	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This could be due to the effect of Mood Disorder on personality .
	manualset3
185060	3	414290	7	NULL	NULL	0	NULL	personality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This could be due to the effect of Mood Disorder on personality .
	manualset3
185061	1	414291	7	NULL	NULL	0	NULL	cross-sectional study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This cross-sectional study aimed to evaluate the prevalence and predictive factors associated with late HIV diagnoses in Houston , Texas using surveillance data .
	manualset3
185062	2	414291	7	NULL	NULL	0	NULL	prevalence factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	This cross-sectional study aimed to evaluate the prevalence and predictive factors associated with late HIV diagnoses in Houston , Texas using surveillance data .
	manualset3
185063	3	414291	7	NULL	NULL	0	NULL	predictive factors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	This cross-sectional study aimed to evaluate the prevalence and predictive factors associated with late HIV diagnoses in Houston , Texas using surveillance data .
	manualset3
185064	4	414291	7	NULL	NULL	0	NULL	late HIV diagnoses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This cross-sectional study aimed to evaluate the prevalence and predictive factors associated with late HIV diagnoses in Houston , Texas using surveillance data .
	manualset3
185065	5	414291	7	NULL	NULL	0	NULL	 Houston	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	This cross-sectional study aimed to evaluate the prevalence and predictive factors associated with late HIV diagnoses in Houston , Texas using surveillance data .
	manualset3
185066	6	414291	7	NULL	NULL	0	NULL	Texas	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	This cross-sectional study aimed to evaluate the prevalence and predictive factors associated with late HIV diagnoses in Houston , Texas using surveillance data .
	manualset3
185067	7	414291	7	NULL	NULL	0	NULL	surveillance data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This cross-sectional study aimed to evaluate the prevalence and predictive factors associated with late HIV diagnoses in Houston , Texas using surveillance data .
	manualset3
185068	1	414292	7	NULL	NULL	NULL	NULL	 current	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This current was found to be involved in the determination of the membrane potential , since glibenclamide depolarized early cardiomyocytes and exerted a positive chronotropic effect .
	manualset3
185069	2	414292	7	NULL	NULL	0	NULL	determination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This current was found to be involved in the determination of the membrane potential , since glibenclamide depolarized early cardiomyocytes and exerted a positive chronotropic effect .
	manualset3
185070	3	414292	7	NULL	NULL	0	NULL	membrane potential	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This current was found to be involved in the determination of the membrane potential , since glibenclamide depolarized early cardiomyocytes and exerted a positive chronotropic effect .
	manualset3
185071	4	414292	7	NULL	NULL	0	NULL	glibenclamide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	This current was found to be involved in the determination of the membrane potential , since glibenclamide depolarized early cardiomyocytes and exerted a positive chronotropic effect .
	manualset3
185072	5	414292	7	NULL	NULL	0	NULL	early cardiomyocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	This current was found to be involved in the determination of the membrane potential , since glibenclamide depolarized early cardiomyocytes and exerted a positive chronotropic effect .
	manualset3
185073	6	414292	7	NULL	NULL	0	NULL	positive chronotropic effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This current was found to be involved in the determination of the membrane potential , since glibenclamide depolarized early cardiomyocytes and exerted a positive chronotropic effect .
	manualset3
185074	1	414293	7	NULL	NULL	0	NULL	cytokine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This cytokine can stimulate production of nitric oxide ( NO ) , via its ability to up-regulate inducible nitric oxide synthase ( iNOS ) .
	manualset3
185075	2	414293	7	NULL	NULL	0	NULL	production 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This cytokine can stimulate production of nitric oxide ( NO ) , via its ability to up-regulate inducible nitric oxide synthase ( iNOS ) .
	manualset3
185076	3	414293	7	NULL	NULL	0	NULL	nitric oxide ( NO )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This cytokine can stimulate production of nitric oxide ( NO ) , via its ability to up-regulate inducible nitric oxide synthase ( iNOS ) .
	manualset3
185077	4	414293	7	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This cytokine can stimulate production of nitric oxide ( NO ) , via its ability to up-regulate inducible nitric oxide synthase ( iNOS ) .
	manualset3
185078	5	414293	7	NULL	NULL	0	NULL	up-regulate	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This cytokine can stimulate production of nitric oxide ( NO ) , via its ability to up-regulate inducible nitric oxide synthase ( iNOS ) .
	manualset3
185079	6	414293	7	NULL	NULL	0	NULL	 inducible nitric oxide synthase ( iNOS )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This cytokine can stimulate production of nitric oxide ( NO ) , via its ability to up-regulate inducible nitric oxide synthase ( iNOS ) .
	manualset3
185080	1	414294	7	NULL	NULL	0	NULL	Adherence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Adherence to treatment guidelines showed remarkable variety among German hospitals , indicating options and need for improvement .
	manualset3
185081	2	414294	7	NULL	NULL	0	NULL	 treatment guidelines	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Adherence to treatment guidelines showed remarkable variety among German hospitals , indicating options and need for improvement .
	manualset3
185082	3	414294	7	NULL	NULL	0	NULL	German hospitals	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Adherence to treatment guidelines showed remarkable variety among German hospitals , indicating options and need for improvement .
	manualset3
185083	4	414294	7	NULL	NULL	0	NULL	improvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Adherence to treatment guidelines showed remarkable variety among German hospitals , indicating options and need for improvement .
	manualset3
185084	1	414295	7	NULL	NULL	0	NULL	damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This damage is potentially lethal , especially in a patient with left main coronary stenosis and previous inferior myocardial infarction .
	manualset3
185085	2	414295	7	NULL	NULL	0	NULL	lethal	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This damage is potentially lethal , especially in a patient with left main coronary stenosis and previous inferior myocardial infarction .
	manualset3
185086	3	414295	7	NULL	NULL	0	NULL	patient	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This damage is potentially lethal , especially in a patient with left main coronary stenosis and previous inferior myocardial infarction .
	manualset3
185087	4	414295	7	NULL	NULL	NULL	NULL	left main coronary stenosis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This damage is potentially lethal , especially in a patient with left main coronary stenosis and previous inferior myocardial infarction .
	manualset3
185088	5	414295	7	NULL	NULL	0	NULL	 inferior myocardial infarction	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This damage is potentially lethal , especially in a patient with left main coronary stenosis and previous inferior myocardial infarction .
	manualset3
185089	1	414296	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This data demonstrates a differential effect of NO signalling on voltage-gated calcium entry , by distinct NO-dependent pathways .
	manualset3
185090	2	414296	7	NULL	NULL	0	NULL	differential effect 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This data demonstrates a differential effect of NO signalling on voltage-gated calcium entry , by distinct NO-dependent pathways .
	manualset3
185091	3	414296	7	NULL	NULL	0	NULL	NO signalling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This data demonstrates a differential effect of NO signalling on voltage-gated calcium entry , by distinct NO-dependent pathways .
	manualset3
185092	4	414296	7	NULL	NULL	0	NULL	voltage-gated calcium entry	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This data demonstrates a differential effect of NO signalling on voltage-gated calcium entry , by distinct NO-dependent pathways .
	manualset3
185093	5	414296	7	NULL	NULL	0	NULL	NO-dependent pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This data demonstrates a differential effect of NO signalling on voltage-gated calcium entry , by distinct NO-dependent pathways .
	manualset3
185094	1	414297	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This data strongly suggest that a short course of antibiotic therapy is efficacious and safe and would result in substantial monetary savings .
	manualset3
185095	2	414297	7	NULL	NULL	0	NULL	short course	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	This data strongly suggest that a short course of antibiotic therapy is efficacious and safe and would result in substantial monetary savings .
	manualset3
185096	3	414297	7	NULL	NULL	0	NULL	antibiotic therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This data strongly suggest that a short course of antibiotic therapy is efficacious and safe and would result in substantial monetary savings .
	manualset3
185097	4	414297	7	NULL	NULL	0	NULL	substantial monetary savings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This data strongly suggest that a short course of antibiotic therapy is efficacious and safe and would result in substantial monetary savings .
	manualset3
185098	1	414298	7	NULL	NULL	0	NULL	decision	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This decision is influenced by various factors such as the dose , the route ( intact vs barrier-disrupted skin ) , the cytokine microenvironment and the nature of the antigenic stimulus .
	manualset3
185099	2	414298	7	NULL	NULL	0	NULL	factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	This decision is influenced by various factors such as the dose , the route ( intact vs barrier-disrupted skin ) , the cytokine microenvironment and the nature of the antigenic stimulus .
	manualset3
185100	3	414298	7	NULL	NULL	0	NULL	dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This decision is influenced by various factors such as the dose , the route ( intact vs barrier-disrupted skin ) , the cytokine microenvironment and the nature of the antigenic stimulus .
	manualset3
185101	4	414298	7	NULL	NULL	0	NULL	 route	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This decision is influenced by various factors such as the dose , the route ( intact vs barrier-disrupted skin ) , the cytokine microenvironment and the nature of the antigenic stimulus .
	manualset3
185102	5	414298	7	NULL	NULL	0	NULL	intact vs barrier-disrupted skin	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This decision is influenced by various factors such as the dose , the route ( intact vs barrier-disrupted skin ) , the cytokine microenvironment and the nature of the antigenic stimulus .
	manualset3
185103	6	414298	7	NULL	NULL	0	NULL	cytokine microenvironment	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	This decision is influenced by various factors such as the dose , the route ( intact vs barrier-disrupted skin ) , the cytokine microenvironment and the nature of the antigenic stimulus .
	manualset3
185104	7	414298	7	NULL	NULL	0	NULL	nature	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	This decision is influenced by various factors such as the dose , the route ( intact vs barrier-disrupted skin ) , the cytokine microenvironment and the nature of the antigenic stimulus .
	manualset3
185105	8	414298	7	NULL	NULL	0	NULL	antigenic stimulus	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This decision is influenced by various factors such as the dose , the route ( intact vs barrier-disrupted skin ) , the cytokine microenvironment and the nature of the antigenic stimulus .
	manualset3
185106	1	414299	7	NULL	NULL	0	NULL	decline 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This decline was transient with recovery of oxidative rates to normal 24 h after MA administration .
	manualset3
185107	2	414299	7	NULL	NULL	0	NULL	recovery	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This decline was transient with recovery of oxidative rates to normal 24 h after MA administration .
	manualset3
185108	3	414299	7	NULL	NULL	0	NULL	oxidative rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This decline was transient with recovery of oxidative rates to normal 24 h after MA administration .
	manualset3
185109	4	414299	7	NULL	NULL	0	NULL	 24 h 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	This decline was transient with recovery of oxidative rates to normal 24 h after MA administration .
	manualset3
185110	5	414299	7	NULL	NULL	0	NULL	MA administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This decline was transient with recovery of oxidative rates to normal 24 h after MA administration .
	manualset3
185111	1	414300	7	NULL	NULL	0	NULL	decrease	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This decrease is accompanied by specific decreases of immunodetected NDA protein and internal rotenone-insensitive NADH oxidation in mitochondria isolated from cold-treated plants .
	manualset3
185112	2	414300	7	NULL	NULL	0	NULL	immunodetected NDA protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This decrease is accompanied by specific decreases of immunodetected NDA protein and internal rotenone-insensitive NADH oxidation in mitochondria isolated from cold-treated plants .
	manualset3
185113	3	414300	7	NULL	NULL	0	NULL	internal rotenone-insensitive NADH oxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This decrease is accompanied by specific decreases of immunodetected NDA protein and internal rotenone-insensitive NADH oxidation in mitochondria isolated from cold-treated plants .
	manualset3
185114	4	414300	7	NULL	NULL	0	NULL	mitochondria	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	This decrease is accompanied by specific decreases of immunodetected NDA protein and internal rotenone-insensitive NADH oxidation in mitochondria isolated from cold-treated plants .
	manualset3
185115	5	414300	7	NULL	NULL	0	NULL	cold-treated plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	This decrease is accompanied by specific decreases of immunodetected NDA protein and internal rotenone-insensitive NADH oxidation in mitochondria isolated from cold-treated plants .
	manualset3
185116	1	414301	7	NULL	NULL	0	NULL	decrease	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This decrease was associated with a suppression of hydrolase activity , suppression of endocytosis , and suppression of oxidative phosphorylation .
	manualset3
185117	2	414301	7	NULL	NULL	0	NULL	suppression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This decrease was associated with a suppression of hydrolase activity , suppression of endocytosis , and suppression of oxidative phosphorylation .
	manualset3
185118	3	414301	7	NULL	NULL	0	NULL	hydrolase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This decrease was associated with a suppression of hydrolase activity , suppression of endocytosis , and suppression of oxidative phosphorylation .
	manualset3
185119	4	414301	7	NULL	NULL	0	NULL	suppression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This decrease was associated with a suppression of hydrolase activity , suppression of endocytosis , and suppression of oxidative phosphorylation .
	manualset3
185120	5	414301	7	NULL	NULL	0	NULL	endocytosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This decrease was associated with a suppression of hydrolase activity , suppression of endocytosis , and suppression of oxidative phosphorylation .
	manualset3
185121	6	414301	7	NULL	NULL	NULL	NULL	suppression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This decrease was associated with a suppression of hydrolase activity , suppression of endocytosis , and suppression of oxidative phosphorylation .
	manualset3
185122	7	414301	7	NULL	NULL	0	NULL	oxidative phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This decrease was associated with a suppression of hydrolase activity , suppression of endocytosis , and suppression of oxidative phosphorylation .
	manualset3
185123	1	414302	7	NULL	NULL	0	NULL	decrease	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This decrease was more pronounced when Al and bepridil were both present in uptake media , but Al did not aggravate verapamil-induced reduction of net ( 45 ) Ca ( 2 + ) uptake .
	manualset3
185124	2	414302	7	NULL	NULL	0	NULL	Al	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This decrease was more pronounced when Al and bepridil were both present in uptake media , but Al did not aggravate verapamil-induced reduction of net ( 45 ) Ca ( 2 + ) uptake .
	manualset3
185125	3	414302	7	NULL	NULL	0	NULL	bepridil 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This decrease was more pronounced when Al and bepridil were both present in uptake media , but Al did not aggravate verapamil-induced reduction of net ( 45 ) Ca ( 2 + ) uptake .
	manualset3
185126	4	414302	7	NULL	NULL	0	NULL	uptake media	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	This decrease was more pronounced when Al and bepridil were both present in uptake media , but Al did not aggravate verapamil-induced reduction of net ( 45 ) Ca ( 2 + ) uptake .
	manualset3
185127	5	414302	7	NULL	NULL	0	NULL	Al	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This decrease was more pronounced when Al and bepridil were both present in uptake media , but Al did not aggravate verapamil-induced reduction of net ( 45 ) Ca ( 2 + ) uptake .
	manualset3
185128	6	414302	7	NULL	NULL	0	NULL	verapamil-induced reduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This decrease was more pronounced when Al and bepridil were both present in uptake media , but Al did not aggravate verapamil-induced reduction of net ( 45 ) Ca ( 2 + ) uptake .
	manualset3
185129	7	414302	7	NULL	NULL	0	NULL	net ( 45 ) Ca ( 2 + ) uptake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This decrease was more pronounced when Al and bepridil were both present in uptake media , but Al did not aggravate verapamil-induced reduction of net ( 45 ) Ca ( 2 + ) uptake .
	manualset3
185130	1	414303	7	NULL	NULL	0	NULL	defect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This defect was largely prevented by hypertonic treatment or overexpression of the dominant-negative 2-W421A-subunit of AP-2 clathrin-adaptor .
	manualset3
185131	2	414303	7	NULL	NULL	0	NULL	hypertonic treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This defect was largely prevented by hypertonic treatment or overexpression of the dominant-negative 2-W421A-subunit of AP-2 clathrin-adaptor .
	manualset3
185132	3	414303	7	NULL	NULL	0	NULL	overexpression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This defect was largely prevented by hypertonic treatment or overexpression of the dominant-negative 2-W421A-subunit of AP-2 clathrin-adaptor .
	manualset3
185133	4	414303	7	NULL	NULL	NULL	NULL	dominant-negative 2-W421A-subunit	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This defect was largely prevented by hypertonic treatment or overexpression of the dominant-negative 2-W421A-subunit of AP-2 clathrin-adaptor .
	manualset3
185134	5	414303	7	NULL	NULL	0	NULL	AP-2 clathrin-adaptor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This defect was largely prevented by hypertonic treatment or overexpression of the dominant-negative 2-W421A-subunit of AP-2 clathrin-adaptor .
	manualset3
185135	1	414304	7	NULL	NULL	NULL	NULL	Adherens junction formation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Adherens junction formation is accompanied by the tyrosine dephosphorylation of adherens junctions proteins , which has been correlated with the strength and stability of adherens junctions .
	manualset3
185136	2	414304	7	NULL	NULL	0	NULL	tyrosine dephosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Adherens junction formation is accompanied by the tyrosine dephosphorylation of adherens junctions proteins , which has been correlated with the strength and stability of adherens junctions .
	manualset3
185137	3	414304	7	NULL	NULL	0	NULL	adherens junctions proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Adherens junction formation is accompanied by the tyrosine dephosphorylation of adherens junctions proteins , which has been correlated with the strength and stability of adherens junctions .
	manualset3
185138	4	414304	7	NULL	NULL	0	NULL	strength	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Adherens junction formation is accompanied by the tyrosine dephosphorylation of adherens junctions proteins , which has been correlated with the strength and stability of adherens junctions .
	manualset3
185139	5	414304	7	NULL	NULL	0	NULL	stability	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Adherens junction formation is accompanied by the tyrosine dephosphorylation of adherens junctions proteins , which has been correlated with the strength and stability of adherens junctions .
	manualset3
185140	6	414304	7	NULL	NULL	0	NULL	adherens junctions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Adherens junction formation is accompanied by the tyrosine dephosphorylation of adherens junctions proteins , which has been correlated with the strength and stability of adherens junctions .
	manualset3
185141	1	414305	7	NULL	NULL	0	NULL	ability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This demonstrates the ability of sHsps to protect cellular proteins , and to maintain cellular viability under conditions of intensive stress , such as heat shock or chemical treatments .
	manualset3
185142	2	414305	7	NULL	NULL	0	NULL	sHsps	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This demonstrates the ability of sHsps to protect cellular proteins , and to maintain cellular viability under conditions of intensive stress , such as heat shock or chemical treatments .
	manualset3
185143	3	414305	7	NULL	NULL	0	NULL	cellular proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This demonstrates the ability of sHsps to protect cellular proteins , and to maintain cellular viability under conditions of intensive stress , such as heat shock or chemical treatments .
	manualset3
185144	4	414305	7	NULL	NULL	0	NULL	cellular viability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This demonstrates the ability of sHsps to protect cellular proteins , and to maintain cellular viability under conditions of intensive stress , such as heat shock or chemical treatments .
	manualset3
185145	5	414305	7	NULL	NULL	0	NULL	conditions 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	This demonstrates the ability of sHsps to protect cellular proteins , and to maintain cellular viability under conditions of intensive stress , such as heat shock or chemical treatments .
	manualset3
185146	6	414305	7	NULL	NULL	NULL	NULL	intensive stress	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This demonstrates the ability of sHsps to protect cellular proteins , and to maintain cellular viability under conditions of intensive stress , such as heat shock or chemical treatments .
	manualset3
185147	7	414305	7	NULL	NULL	NULL	NULL	heat shock treatments	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This demonstrates the ability of sHsps to protect cellular proteins , and to maintain cellular viability under conditions of intensive stress , such as heat shock or chemical treatments .
	manualset3
185148	8	414305	7	NULL	NULL	NULL	NULL	chemical treatments	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This demonstrates the ability of sHsps to protect cellular proteins , and to maintain cellular viability under conditions of intensive stress , such as heat shock or chemical treatments .
	manualset3
185149	1	414306	7	NULL	NULL	0	NULL	desensitization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This desensitization was shown not to involve activation of protein kinase C .
	manualset3
185268	2	414306	7	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This desensitization was shown not to involve activation of protein kinase C .
	manualset3
185269	3	414306	7	NULL	NULL	0	NULL	protein kinase C	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This desensitization was shown not to involve activation of protein kinase C .
	manualset3
185277	1	414307	7	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference could be attributed to a decline in IF IgG antibody with time after infection .
	manualset3
185278	2	414307	7	NULL	NULL	0	NULL	 decline	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference could be attributed to a decline in IF IgG antibody with time after infection .
	manualset3
185279	3	414307	7	NULL	NULL	NULL	NULL	IF IgG antibody	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This difference could be attributed to a decline in IF IgG antibody with time after infection .
	manualset3
185280	4	414307	7	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference could be attributed to a decline in IF IgG antibody with time after infection .
	manualset3
185281	5	414307	7	NULL	NULL	0	NULL	infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference could be attributed to a decline in IF IgG antibody with time after infection .
	manualset3
185282	1	414308	7	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was accounted for by significantly smaller left and right STG white matter volumes in bipolar patients .
	manualset3
185283	2	414308	7	NULL	NULL	NULL	NULL	 smaller left white matter volumes	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This difference was accounted for by significantly smaller left and right STG white matter volumes in bipolar patients .
	manualset3
185284	3	414308	7	NULL	NULL	0	NULL	 right STG white matter volumes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was accounted for by significantly smaller left and right STG white matter volumes in bipolar patients .
	manualset3
185285	4	414308	7	NULL	NULL	0	NULL	bipolar patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was accounted for by significantly smaller left and right STG white matter volumes in bipolar patients .
	manualset3
185286	1	414309	7	NULL	NULL	0	NULL	 difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was due to the higher incidence of responses with latencies between 2.7 and 10 msec outside of the SSN ( 44 % ) compared to SSN responses ( 8 % ) .
	manualset3
185287	2	414309	7	NULL	NULL	0	NULL	higher incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was due to the higher incidence of responses with latencies between 2.7 and 10 msec outside of the SSN ( 44 % ) compared to SSN responses ( 8 % ) .
	manualset3
185288	3	414309	7	NULL	NULL	0	NULL	responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was due to the higher incidence of responses with latencies between 2.7 and 10 msec outside of the SSN ( 44 % ) compared to SSN responses ( 8 % ) .
	manualset3
185289	4	414309	7	NULL	NULL	0	NULL	2.7 msec	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was due to the higher incidence of responses with latencies between 2.7 and 10 msec outside of the SSN ( 44 % ) compared to SSN responses ( 8 % ) .
	manualset3
185290	5	414309	7	NULL	NULL	0	NULL	10 msec	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was due to the higher incidence of responses with latencies between 2.7 and 10 msec outside of the SSN ( 44 % ) compared to SSN responses ( 8 % ) .
	manualset3
185296	6	414309	7	NULL	NULL	0	NULL	SSN responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was due to the higher incidence of responses with latencies between 2.7 and 10 msec outside of the SSN ( 44 % ) compared to SSN responses ( 8 % ) .
	manualset3
185297	7	414309	7	NULL	NULL	0	NULL	44 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was due to the higher incidence of responses with latencies between 2.7 and 10 msec outside of the SSN ( 44 % ) compared to SSN responses ( 8 % ) .
	manualset3
185298	8	414309	7	NULL	NULL	0	NULL	SSN responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was due to the higher incidence of responses with latencies between 2.7 and 10 msec outside of the SSN ( 44 % ) compared to SSN responses ( 8 % ) .
	manualset3
185302	9	414309	7	NULL	NULL	0	NULL	 8 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was due to the higher incidence of responses with latencies between 2.7 and 10 msec outside of the SSN ( 44 % ) compared to SSN responses ( 8 % ) .
	manualset3
185303	10	414309	7	NULL	NULL	0	NULL	latencies	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was due to the higher incidence of responses with latencies between 2.7 and 10 msec outside of the SSN ( 44 % ) compared to SSN responses ( 8 % ) .
	manualset3
185304	11	414309	7	NULL	NULL	0	NULL	outside	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was due to the higher incidence of responses with latencies between 2.7 and 10 msec outside of the SSN ( 44 % ) compared to SSN responses ( 8 % ) .
	manualset3
185305	1	414310	7	NULL	NULL	0	NULL	difference 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was entirely due to an increase in SMC number within the intima .
	manualset3
185306	2	414310	7	NULL	NULL	0	NULL	increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was entirely due to an increase in SMC number within the intima .
	manualset3
185307	3	414310	7	NULL	NULL	0	NULL	SMC number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was entirely due to an increase in SMC number within the intima .
	manualset3
185308	4	414310	7	NULL	NULL	0	NULL	 intima	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was entirely due to an increase in SMC number within the intima .
	manualset3
185309	1	414311	7	NULL	NULL	0	NULL	Comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparison between the electroneurographic effects of gustatory activation of Staderini 's nucleus intercalatus and of those of adjacent bulbar regions ) .
	manualset3
185310	2	414311	7	NULL	NULL	0	NULL	electroneurographic effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparison between the electroneurographic effects of gustatory activation of Staderini 's nucleus intercalatus and of those of adjacent bulbar regions ) .
	manualset3
185311	3	414311	7	NULL	NULL	0	NULL	gustatory activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparison between the electroneurographic effects of gustatory activation of Staderini 's nucleus intercalatus and of those of adjacent bulbar regions ) .
	manualset3
185312	4	414311	7	NULL	NULL	0	NULL	Staderini 's nucleus intercalatus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparison between the electroneurographic effects of gustatory activation of Staderini 's nucleus intercalatus and of those of adjacent bulbar regions ) .
	manualset3
185313	5	414311	7	NULL	NULL	0	NULL	adjacent bulbar regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Comparison between the electroneurographic effects of gustatory activation of Staderini 's nucleus intercalatus and of those of adjacent bulbar regions ) .
	manualset3
185314	1	414312	7	NULL	NULL	NULL	NULL	Adherents 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Adherents of a countertrend have long suggested the importance of analysis of HLA haplotypes ( combinations of alleles on 1 chromosome ) rather than individual genes .
	manualset3
185315	2	414312	7	NULL	NULL	NULL	NULL	countertrend	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Adherents of a countertrend have long suggested the importance of analysis of HLA haplotypes ( combinations of alleles on 1 chromosome ) rather than individual genes .
	manualset3
185316	3	414312	7	NULL	NULL	NULL	NULL	analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Adherents of a countertrend have long suggested the importance of analysis of HLA haplotypes ( combinations of alleles on 1 chromosome ) rather than individual genes .
	manualset3
185317	4	414312	7	NULL	NULL	0	NULL	HLA haplotypes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Adherents of a countertrend have long suggested the importance of analysis of HLA haplotypes ( combinations of alleles on 1 chromosome ) rather than individual genes .
	manualset3
185318	5	414312	7	NULL	NULL	NULL	NULL	combinations of alleles	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Adherents of a countertrend have long suggested the importance of analysis of HLA haplotypes ( combinations of alleles on 1 chromosome ) rather than individual genes .
	manualset3
185320	7	414312	7	NULL	NULL	0	NULL	1 chromosome	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Adherents of a countertrend have long suggested the importance of analysis of HLA haplotypes ( combinations of alleles on 1 chromosome ) rather than individual genes .
	manualset3
185321	8	414312	7	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Adherents of a countertrend have long suggested the importance of analysis of HLA haplotypes ( combinations of alleles on 1 chromosome ) rather than individual genes .
	manualset3
185322	1	414313	7	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was more pronounced in the subset of patients with seminal vesicle invasion : 30 % local recurrence in the surgery only group versus 0 in the irradiated group .
	manualset3
185323	2	414313	7	NULL	NULL	0	NULL	subset of patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was more pronounced in the subset of patients with seminal vesicle invasion : 30 % local recurrence in the surgery only group versus 0 in the irradiated group .
	manualset3
185324	3	414313	7	NULL	NULL	0	NULL	seminal vesicle invasion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was more pronounced in the subset of patients with seminal vesicle invasion : 30 % local recurrence in the surgery only group versus 0 in the irradiated group .
	manualset3
185325	4	414313	7	NULL	NULL	0	NULL	30 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was more pronounced in the subset of patients with seminal vesicle invasion : 30 % local recurrence in the surgery only group versus 0 in the irradiated group .
	manualset3
185326	5	414313	7	NULL	NULL	NULL	NULL	local recurrence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This difference was more pronounced in the subset of patients with seminal vesicle invasion : 30 % local recurrence in the surgery only group versus 0 in the irradiated group .
	manualset3
185327	6	414313	7	NULL	NULL	0	NULL	surgery only group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was more pronounced in the subset of patients with seminal vesicle invasion : 30 % local recurrence in the surgery only group versus 0 in the irradiated group .
	manualset3
185328	7	414313	7	NULL	NULL	NULL	NULL	0 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This difference was more pronounced in the subset of patients with seminal vesicle invasion : 30 % local recurrence in the surgery only group versus 0 in the irradiated group .
	manualset3
185329	8	414313	7	NULL	NULL	0	NULL	 irradiated group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was more pronounced in the subset of patients with seminal vesicle invasion : 30 % local recurrence in the surgery only group versus 0 in the irradiated group .
	manualset3
185330	1	414314	7	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was statistically significant , and provided the opportunity to compare activity levels of the monkeys over two dietary periods , one characterized primarily by folivory , the other by frugivory .
	manualset3
185331	2	414314	7	NULL	NULL	0	NULL	opportunity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was statistically significant , and provided the opportunity to compare activity levels of the monkeys over two dietary periods , one characterized primarily by folivory , the other by frugivory .
	manualset3
185332	3	414314	7	NULL	NULL	0	NULL	activity levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was statistically significant , and provided the opportunity to compare activity levels of the monkeys over two dietary periods , one characterized primarily by folivory , the other by frugivory .
	manualset3
185333	4	414314	7	NULL	NULL	0	NULL	monkeys	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was statistically significant , and provided the opportunity to compare activity levels of the monkeys over two dietary periods , one characterized primarily by folivory , the other by frugivory .
	manualset3
185334	5	414314	7	NULL	NULL	0	NULL	two dietary periods	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was statistically significant , and provided the opportunity to compare activity levels of the monkeys over two dietary periods , one characterized primarily by folivory , the other by frugivory .
	manualset3
185335	6	414314	7	NULL	NULL	0	NULL	 one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was statistically significant , and provided the opportunity to compare activity levels of the monkeys over two dietary periods , one characterized primarily by folivory , the other by frugivory .
	manualset3
185336	7	414314	7	NULL	NULL	0	NULL	 folivory	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was statistically significant , and provided the opportunity to compare activity levels of the monkeys over two dietary periods , one characterized primarily by folivory , the other by frugivory .
	manualset3
185337	8	414314	7	NULL	NULL	0	NULL	frugivory	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was statistically significant , and provided the opportunity to compare activity levels of the monkeys over two dietary periods , one characterized primarily by folivory , the other by frugivory .
	manualset3
185338	1	414315	7	NULL	NULL	0	NULL	difference 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was statistically significant only at the first evaluation ( i.e. before the combined norgestimate regimen ) and was not observed in the 4th cycle ( i.e. during the Cileste regimen ) , while the incidence of menstrual disturbances was generally found to decrease .
	manualset3
185339	2	414315	7	NULL	NULL	0	NULL	first evaluation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was statistically significant only at the first evaluation ( i.e. before the combined norgestimate regimen ) and was not observed in the 4th cycle ( i.e. during the Cileste regimen ) , while the incidence of menstrual disturbances was generally found to decrease .
	manualset3
185340	3	414315	7	NULL	NULL	0	NULL	combined norgestimate regimen	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was statistically significant only at the first evaluation ( i.e. before the combined norgestimate regimen ) and was not observed in the 4th cycle ( i.e. during the Cileste regimen ) , while the incidence of menstrual disturbances was generally found to decrease .
	manualset3
185341	4	414315	7	NULL	NULL	0	NULL	4th cycle 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was statistically significant only at the first evaluation ( i.e. before the combined norgestimate regimen ) and was not observed in the 4th cycle ( i.e. during the Cileste regimen ) , while the incidence of menstrual disturbances was generally found to decrease .
	manualset3
185342	5	414315	7	NULL	NULL	0	NULL	 Cileste regimen 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was statistically significant only at the first evaluation ( i.e. before the combined norgestimate regimen ) and was not observed in the 4th cycle ( i.e. during the Cileste regimen ) , while the incidence of menstrual disturbances was generally found to decrease .
	manualset3
185343	6	414315	7	NULL	NULL	0	NULL	 incidence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was statistically significant only at the first evaluation ( i.e. before the combined norgestimate regimen ) and was not observed in the 4th cycle ( i.e. during the Cileste regimen ) , while the incidence of menstrual disturbances was generally found to decrease .
	manualset3
185344	7	414315	7	NULL	NULL	0	NULL	menstrual disturbances	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This difference was statistically significant only at the first evaluation ( i.e. before the combined norgestimate regimen ) and was not observed in the 4th cycle ( i.e. during the Cileste regimen ) , while the incidence of menstrual disturbances was generally found to decrease .
	manualset3
185353	1	414316	7	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This differentiation correlated with reduction in proliferation and limited migration of the donor cells within the regenerating muscle .
	manualset3
185354	2	414316	7	NULL	NULL	0	NULL	reduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This differentiation correlated with reduction in proliferation and limited migration of the donor cells within the regenerating muscle .
	manualset3
185355	3	414316	7	NULL	NULL	0	NULL	proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This differentiation correlated with reduction in proliferation and limited migration of the donor cells within the regenerating muscle .
	manualset3
185356	4	414316	7	NULL	NULL	0	NULL	 limited migration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This differentiation correlated with reduction in proliferation and limited migration of the donor cells within the regenerating muscle .
	manualset3
185357	5	414316	7	NULL	NULL	0	NULL	donor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	This differentiation correlated with reduction in proliferation and limited migration of the donor cells within the regenerating muscle .
	manualset3
185358	6	414316	7	NULL	NULL	0	NULL	 regenerating muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This differentiation correlated with reduction in proliferation and limited migration of the donor cells within the regenerating muscle .
	manualset3
185359	1	414317	7	NULL	NULL	0	NULL	discussion paper 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This discussion paper argues for the critical importance of successful leadership for effective mental health nursing , observing that nursing leadership has long been regarded problematically by the profession .
	manualset3
185360	2	414317	7	NULL	NULL	0	NULL	 leadership	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This discussion paper argues for the critical importance of successful leadership for effective mental health nursing , observing that nursing leadership has long been regarded problematically by the profession .
	manualset3
185362	3	414317	7	NULL	NULL	0	NULL	effective mental health nursing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This discussion paper argues for the critical importance of successful leadership for effective mental health nursing , observing that nursing leadership has long been regarded problematically by the profession .
	manualset3
185363	4	414317	7	NULL	NULL	0	NULL	observing 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This discussion paper argues for the critical importance of successful leadership for effective mental health nursing , observing that nursing leadership has long been regarded problematically by the profession .
	manualset3
185367	5	414317	7	NULL	NULL	0	NULL	nursing leadership	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This discussion paper argues for the critical importance of successful leadership for effective mental health nursing , observing that nursing leadership has long been regarded problematically by the profession .
	manualset3
185369	6	414317	7	NULL	NULL	0	NULL	profession	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This discussion paper argues for the critical importance of successful leadership for effective mental health nursing , observing that nursing leadership has long been regarded problematically by the profession .
	manualset3
185372	1	414318	7	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This disease affects postmenopausal women most frequently , and a link clearly exists between estrogen deficiency and accelerated bone loss .
	manualset3
185374	2	414318	7	NULL	NULL	0	NULL	postmenopausal women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This disease affects postmenopausal women most frequently , and a link clearly exists between estrogen deficiency and accelerated bone loss .
	manualset3
185377	3	414318	7	NULL	NULL	0	NULL	link 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	This disease affects postmenopausal women most frequently , and a link clearly exists between estrogen deficiency and accelerated bone loss .
	manualset3
185380	4	414318	7	NULL	NULL	0	NULL	estrogen deficiency 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This disease affects postmenopausal women most frequently , and a link clearly exists between estrogen deficiency and accelerated bone loss .
	manualset3
185381	5	414318	7	NULL	NULL	0	NULL	accelerated bone loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This disease affects postmenopausal women most frequently , and a link clearly exists between estrogen deficiency and accelerated bone loss .
	manualset3
185387	1	414319	7	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This disease was confirmed ultrastructurally by demonstration of typical adenoviral particles in the nuclei of endothelial cells in the myocardium and of interstitial cells in the small intestine .
	manualset3
185388	2	414319	7	NULL	NULL	0	NULL	demonstration	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This disease was confirmed ultrastructurally by demonstration of typical adenoviral particles in the nuclei of endothelial cells in the myocardium and of interstitial cells in the small intestine .
	manualset3
185390	3	414319	7	NULL	NULL	0	NULL	adenoviral particles	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	This disease was confirmed ultrastructurally by demonstration of typical adenoviral particles in the nuclei of endothelial cells in the myocardium and of interstitial cells in the small intestine .
	manualset3
185393	4	414319	7	NULL	NULL	0	NULL	nuclei	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	This disease was confirmed ultrastructurally by demonstration of typical adenoviral particles in the nuclei of endothelial cells in the myocardium and of interstitial cells in the small intestine .
	manualset3
185396	5	414319	7	NULL	NULL	0	NULL	endothelial cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	This disease was confirmed ultrastructurally by demonstration of typical adenoviral particles in the nuclei of endothelial cells in the myocardium and of interstitial cells in the small intestine .
	manualset3
185397	6	414319	7	NULL	NULL	0	NULL	myocardium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This disease was confirmed ultrastructurally by demonstration of typical adenoviral particles in the nuclei of endothelial cells in the myocardium and of interstitial cells in the small intestine .
	manualset3
185398	7	414319	7	NULL	NULL	0	NULL	interstitial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	This disease was confirmed ultrastructurally by demonstration of typical adenoviral particles in the nuclei of endothelial cells in the myocardium and of interstitial cells in the small intestine .
	manualset3
185399	8	414319	7	NULL	NULL	0	NULL	small intestine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This disease was confirmed ultrastructurally by demonstration of typical adenoviral particles in the nuclei of endothelial cells in the myocardium and of interstitial cells in the small intestine .
	manualset3
185400	1	414320	7	NULL	NULL	0	NULL	diversity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This diversity , resulting from both amino acid and glycan heterogeneity , is translated into cellular responses through Fc receptors ( FcRs ) , a structurally and functionally diverse family of cell surface receptors found throughout the immune system .
	manualset3
185401	2	414320	7	NULL	NULL	0	NULL	amino acid	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	This diversity , resulting from both amino acid and glycan heterogeneity , is translated into cellular responses through Fc receptors ( FcRs ) , a structurally and functionally diverse family of cell surface receptors found throughout the immune system .
	manualset3
185402	3	414320	7	NULL	NULL	0	NULL	glycan heterogeneity	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This diversity , resulting from both amino acid and glycan heterogeneity , is translated into cellular responses through Fc receptors ( FcRs ) , a structurally and functionally diverse family of cell surface receptors found throughout the immune system .
	manualset3
185403	4	414320	7	NULL	NULL	0	NULL	cellular responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This diversity , resulting from both amino acid and glycan heterogeneity , is translated into cellular responses through Fc receptors ( FcRs ) , a structurally and functionally diverse family of cell surface receptors found throughout the immune system .
	manualset3
185404	5	414320	7	NULL	NULL	0	NULL	Fc receptors ( FcRs )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This diversity , resulting from both amino acid and glycan heterogeneity , is translated into cellular responses through Fc receptors ( FcRs ) , a structurally and functionally diverse family of cell surface receptors found throughout the immune system .
	manualset3
185406	6	414320	7	NULL	NULL	0	NULL	 family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This diversity , resulting from both amino acid and glycan heterogeneity , is translated into cellular responses through Fc receptors ( FcRs ) , a structurally and functionally diverse family of cell surface receptors found throughout the immune system .
	manualset3
185408	7	414320	7	NULL	NULL	0	NULL	cell surface receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This diversity , resulting from both amino acid and glycan heterogeneity , is translated into cellular responses through Fc receptors ( FcRs ) , a structurally and functionally diverse family of cell surface receptors found throughout the immune system .
	manualset3
185409	8	414320	7	NULL	NULL	0	NULL	immune system 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This diversity , resulting from both amino acid and glycan heterogeneity , is translated into cellular responses through Fc receptors ( FcRs ) , a structurally and functionally diverse family of cell surface receptors found throughout the immune system .
	manualset3
185507	1	414321	7	NULL	NULL	0	NULL	 diversity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This diversity could be due to drift , as indicated by the neutrality test performed .
	manualset3
185508	2	414321	7	NULL	NULL	0	NULL	drift	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This diversity could be due to drift , as indicated by the neutrality test performed .
	manualset3
185509	3	414321	7	NULL	NULL	0	NULL	neutrality test	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This diversity could be due to drift , as indicated by the neutrality test performed .
	manualset3
185510	1	414322	7	NULL	NULL	0	NULL	Adhesion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Adhesion , apoptosis and cytokine release of human mononuclear cells cultured on degradable poly ( urethane urea ) , polystyrene and titanium in vitro .
	manualset3
185511	2	414322	7	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Adhesion , apoptosis and cytokine release of human mononuclear cells cultured on degradable poly ( urethane urea ) , polystyrene and titanium in vitro .
	manualset3
185512	3	414322	7	NULL	NULL	0	NULL	cytokine release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Adhesion , apoptosis and cytokine release of human mononuclear cells cultured on degradable poly ( urethane urea ) , polystyrene and titanium in vitro .
	manualset3
185513	4	414322	7	NULL	NULL	0	NULL	human mononuclear cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Adhesion , apoptosis and cytokine release of human mononuclear cells cultured on degradable poly ( urethane urea ) , polystyrene and titanium in vitro .
	manualset3
185514	5	414322	7	NULL	NULL	0	NULL	poly ( urethane urea )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Adhesion , apoptosis and cytokine release of human mononuclear cells cultured on degradable poly ( urethane urea ) , polystyrene and titanium in vitro .
	manualset3
185515	6	414322	7	NULL	NULL	0	NULL	polystyrene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Adhesion , apoptosis and cytokine release of human mononuclear cells cultured on degradable poly ( urethane urea ) , polystyrene and titanium in vitro .
	manualset3
185516	7	414322	7	NULL	NULL	0	NULL	titanium 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Adhesion , apoptosis and cytokine release of human mononuclear cells cultured on degradable poly ( urethane urea ) , polystyrene and titanium in vitro .
	manualset3
185517	1	414323	7	NULL	NULL	0	NULL	broad band	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This does not imply a broad band of co-resistance to different stress types but reflects a continuous cross talk during the coevolution of plants , pathogens and herbivores competing in an environment where efficient metal ion acquisition and ion homeostasis are essential for survival .
	manualset3
185518	2	414323	7	NULL	NULL	0	NULL	co-resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This does not imply a broad band of co-resistance to different stress types but reflects a continuous cross talk during the coevolution of plants , pathogens and herbivores competing in an environment where efficient metal ion acquisition and ion homeostasis are essential for survival .
	manualset3
185519	3	414323	7	NULL	NULL	0	NULL	stress types	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This does not imply a broad band of co-resistance to different stress types but reflects a continuous cross talk during the coevolution of plants , pathogens and herbivores competing in an environment where efficient metal ion acquisition and ion homeostasis are essential for survival .
	manualset3
185520	4	414323	7	NULL	NULL	0	NULL	continuous cross talk	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This does not imply a broad band of co-resistance to different stress types but reflects a continuous cross talk during the coevolution of plants , pathogens and herbivores competing in an environment where efficient metal ion acquisition and ion homeostasis are essential for survival .
	manualset3
185521	5	414323	7	NULL	NULL	0	NULL	coevolution 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This does not imply a broad band of co-resistance to different stress types but reflects a continuous cross talk during the coevolution of plants , pathogens and herbivores competing in an environment where efficient metal ion acquisition and ion homeostasis are essential for survival .
	manualset3
185522	6	414323	7	NULL	NULL	0	NULL	plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	This does not imply a broad band of co-resistance to different stress types but reflects a continuous cross talk during the coevolution of plants , pathogens and herbivores competing in an environment where efficient metal ion acquisition and ion homeostasis are essential for survival .
	manualset3
185523	7	414323	7	NULL	NULL	0	NULL	pathogens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	This does not imply a broad band of co-resistance to different stress types but reflects a continuous cross talk during the coevolution of plants , pathogens and herbivores competing in an environment where efficient metal ion acquisition and ion homeostasis are essential for survival .
	manualset3
185524	8	414323	7	NULL	NULL	0	NULL	herbivores	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	This does not imply a broad band of co-resistance to different stress types but reflects a continuous cross talk during the coevolution of plants , pathogens and herbivores competing in an environment where efficient metal ion acquisition and ion homeostasis are essential for survival .
	manualset3
185525	9	414323	7	NULL	NULL	0	NULL	environment	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	This does not imply a broad band of co-resistance to different stress types but reflects a continuous cross talk during the coevolution of plants , pathogens and herbivores competing in an environment where efficient metal ion acquisition and ion homeostasis are essential for survival .
	manualset3
185526	10	414323	7	NULL	NULL	0	NULL	metal ion acquisition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This does not imply a broad band of co-resistance to different stress types but reflects a continuous cross talk during the coevolution of plants , pathogens and herbivores competing in an environment where efficient metal ion acquisition and ion homeostasis are essential for survival .
	manualset3
185527	11	414323	7	NULL	NULL	0	NULL	ion homeostasis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This does not imply a broad band of co-resistance to different stress types but reflects a continuous cross talk during the coevolution of plants , pathogens and herbivores competing in an environment where efficient metal ion acquisition and ion homeostasis are essential for survival .
	manualset3
185528	12	414323	7	NULL	NULL	0	NULL	survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This does not imply a broad band of co-resistance to different stress types but reflects a continuous cross talk during the coevolution of plants , pathogens and herbivores competing in an environment where efficient metal ion acquisition and ion homeostasis are essential for survival .
	manualset3
185529	1	414324	7	NULL	NULL	NULL	NULL	dosage	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This dosage of aspirin does not affect the hypotensive activity of arachidonic acid nor the oedematous properties of carrageenan in the rat .
	manualset3
185530	2	414324	7	NULL	NULL	0	NULL	aspirin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	This dosage of aspirin does not affect the hypotensive activity of arachidonic acid nor the oedematous properties of carrageenan in the rat .
	manualset3
185531	3	414324	7	NULL	NULL	0	NULL	hypotensive activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This dosage of aspirin does not affect the hypotensive activity of arachidonic acid nor the oedematous properties of carrageenan in the rat .
	manualset3
185532	4	414324	7	NULL	NULL	0	NULL	arachidonic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This dosage of aspirin does not affect the hypotensive activity of arachidonic acid nor the oedematous properties of carrageenan in the rat .
	manualset3
185533	5	414324	7	NULL	NULL	0	NULL	oedematous properties	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This dosage of aspirin does not affect the hypotensive activity of arachidonic acid nor the oedematous properties of carrageenan in the rat .
	manualset3
185534	6	414324	7	NULL	NULL	0	NULL	carrageenan	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This dosage of aspirin does not affect the hypotensive activity of arachidonic acid nor the oedematous properties of carrageenan in the rat .
	manualset3
185535	7	414324	7	NULL	NULL	0	NULL	rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	This dosage of aspirin does not affect the hypotensive activity of arachidonic acid nor the oedematous properties of carrageenan in the rat .
	manualset3
185536	1	414325	7	NULL	NULL	0	NULL	double-negative mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This double-negative mechanism , together with direct activation via the achaete enhancer , increases expression of achaete and ensures robust development of sensory neurons .
	manualset3
185537	2	414325	7	NULL	NULL	0	NULL	direct activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This double-negative mechanism , together with direct activation via the achaete enhancer , increases expression of achaete and ensures robust development of sensory neurons .
	manualset3
185538	3	414325	7	NULL	NULL	0	NULL	achaete enhancer	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This double-negative mechanism , together with direct activation via the achaete enhancer , increases expression of achaete and ensures robust development of sensory neurons .
	manualset3
185539	4	414325	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This double-negative mechanism , together with direct activation via the achaete enhancer , increases expression of achaete and ensures robust development of sensory neurons .
	manualset3
185540	5	414325	7	NULL	NULL	0	NULL	achaete	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This double-negative mechanism , together with direct activation via the achaete enhancer , increases expression of achaete and ensures robust development of sensory neurons .
	manualset3
185541	6	414325	7	NULL	NULL	0	NULL	development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This double-negative mechanism , together with direct activation via the achaete enhancer , increases expression of achaete and ensures robust development of sensory neurons .
	manualset3
185542	7	414325	7	NULL	NULL	NULL	NULL	 sensory neurons	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This double-negative mechanism , together with direct activation via the achaete enhancer , increases expression of achaete and ensures robust development of sensory neurons .
	manualset3
189773	8	414325	7	NULL	NULL	0	NULL	achaete enhancer	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	This double-negative mechanism , together with direct activation via the achaete enhancer , increases expression of achaete and ensures robust development of sensory neurons .
	manualset3
185543	1	414326	7	NULL	NULL	0	NULL	double blind cross over study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This double blind cross over study comparing triazolam and nitrazepam conducted by G.P. 's on insomniacs is the first French clinical study intended for the registration application and done according to this methodology .
	manualset3
185544	2	414326	7	NULL	NULL	0	NULL	triazolam	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	This double blind cross over study comparing triazolam and nitrazepam conducted by G.P. 's on insomniacs is the first French clinical study intended for the registration application and done according to this methodology .
	manualset3
185545	3	414326	7	NULL	NULL	0	NULL	nitrazepam	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	This double blind cross over study comparing triazolam and nitrazepam conducted by G.P. 's on insomniacs is the first French clinical study intended for the registration application and done according to this methodology .
	manualset3
185546	4	414326	7	NULL	NULL	0	NULL	G.P. 's	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This double blind cross over study comparing triazolam and nitrazepam conducted by G.P. 's on insomniacs is the first French clinical study intended for the registration application and done according to this methodology .
	manualset3
185547	5	414326	7	NULL	NULL	0	NULL	insomniacs	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This double blind cross over study comparing triazolam and nitrazepam conducted by G.P. 's on insomniacs is the first French clinical study intended for the registration application and done according to this methodology .
	manualset3
185548	6	414326	7	NULL	NULL	0	NULL	first French clinical study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This double blind cross over study comparing triazolam and nitrazepam conducted by G.P. 's on insomniacs is the first French clinical study intended for the registration application and done according to this methodology .
	manualset3
185549	7	414326	7	NULL	NULL	0	NULL	registration application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This double blind cross over study comparing triazolam and nitrazepam conducted by G.P. 's on insomniacs is the first French clinical study intended for the registration application and done according to this methodology .
	manualset3
185550	8	414326	7	NULL	NULL	0	NULL	methodology 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This double blind cross over study comparing triazolam and nitrazepam conducted by G.P. 's on insomniacs is the first French clinical study intended for the registration application and done according to this methodology .
	manualset3
185551	1	414327	7	NULL	NULL	0	NULL	 drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	This drug exhibited favourable properties as a photosensitizer in vitro because ZnPcOCH ( 3 ) is able to penetrate efficiently in the cytoplasm of cultured cancer cells and is partially localized in lysosomes .
	manualset3
185552	2	414327	7	NULL	NULL	0	NULL	 properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	This drug exhibited favourable properties as a photosensitizer in vitro because ZnPcOCH ( 3 ) is able to penetrate efficiently in the cytoplasm of cultured cancer cells and is partially localized in lysosomes .
	manualset3
185553	3	414327	7	NULL	NULL	0	NULL	photosensitizer	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	This drug exhibited favourable properties as a photosensitizer in vitro because ZnPcOCH ( 3 ) is able to penetrate efficiently in the cytoplasm of cultured cancer cells and is partially localized in lysosomes .
	manualset3
185554	4	414327	7	NULL	NULL	0	NULL	ZnPcOCH ( 3 ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This drug exhibited favourable properties as a photosensitizer in vitro because ZnPcOCH ( 3 ) is able to penetrate efficiently in the cytoplasm of cultured cancer cells and is partially localized in lysosomes .
	manualset3
185555	5	414327	7	NULL	NULL	0	NULL	cytoplasm	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	This drug exhibited favourable properties as a photosensitizer in vitro because ZnPcOCH ( 3 ) is able to penetrate efficiently in the cytoplasm of cultured cancer cells and is partially localized in lysosomes .
	manualset3
185556	6	414327	7	NULL	NULL	NULL	NULL	cultured cancer cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This drug exhibited favourable properties as a photosensitizer in vitro because ZnPcOCH ( 3 ) is able to penetrate efficiently in the cytoplasm of cultured cancer cells and is partially localized in lysosomes .
	manualset3
185557	7	414327	7	NULL	NULL	0	NULL	lysosomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	This drug exhibited favourable properties as a photosensitizer in vitro because ZnPcOCH ( 3 ) is able to penetrate efficiently in the cytoplasm of cultured cancer cells and is partially localized in lysosomes .
	manualset3
185558	1	414328	7	NULL	NULL	0	NULL	effect 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This effect has important influence on the amount of the resultant .
	manualset3
185559	2	414328	7	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This effect has important influence on the amount of the resultant .
	manualset3
185560	3	414328	7	NULL	NULL	0	NULL	resultant	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	This effect has important influence on the amount of the resultant .
	manualset3
185561	1	414329	7	NULL	NULL	NULL	NULL	 effect 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This effect is caused by a noncooperative interaction of water molecules with electrophilic groups of amino acid and by intramolecular hydrogen bond , allowing proton transfer from the carboxylic to the amine group , accomplishing by the chain of two to four water molecules .
	manualset3
185562	2	414329	7	NULL	NULL	0	NULL	 noncooperative interaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This effect is caused by a noncooperative interaction of water molecules with electrophilic groups of amino acid and by intramolecular hydrogen bond , allowing proton transfer from the carboxylic to the amine group , accomplishing by the chain of two to four water molecules .
	manualset3
185563	3	414329	7	NULL	NULL	0	NULL	water molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	This effect is caused by a noncooperative interaction of water molecules with electrophilic groups of amino acid and by intramolecular hydrogen bond , allowing proton transfer from the carboxylic to the amine group , accomplishing by the chain of two to four water molecules .
	manualset3
185564	4	414329	7	NULL	NULL	0	NULL	electrophilic groups	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	This effect is caused by a noncooperative interaction of water molecules with electrophilic groups of amino acid and by intramolecular hydrogen bond , allowing proton transfer from the carboxylic to the amine group , accomplishing by the chain of two to four water molecules .
	manualset3
185565	5	414329	7	NULL	NULL	0	NULL	amino acid	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	This effect is caused by a noncooperative interaction of water molecules with electrophilic groups of amino acid and by intramolecular hydrogen bond , allowing proton transfer from the carboxylic to the amine group , accomplishing by the chain of two to four water molecules .
	manualset3
185566	6	414329	7	NULL	NULL	0	NULL	intramolecular hydrogen bond 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This effect is caused by a noncooperative interaction of water molecules with electrophilic groups of amino acid and by intramolecular hydrogen bond , allowing proton transfer from the carboxylic to the amine group , accomplishing by the chain of two to four water molecules .
	manualset3
185567	7	414329	7	NULL	NULL	0	NULL	proton transfer	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This effect is caused by a noncooperative interaction of water molecules with electrophilic groups of amino acid and by intramolecular hydrogen bond , allowing proton transfer from the carboxylic to the amine group , accomplishing by the chain of two to four water molecules .
	manualset3
185568	8	414329	7	NULL	NULL	NULL	NULL	carboxylic group	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This effect is caused by a noncooperative interaction of water molecules with electrophilic groups of amino acid and by intramolecular hydrogen bond , allowing proton transfer from the carboxylic to the amine group , accomplishing by the chain of two to four water molecules .
	manualset3
185569	9	414329	7	NULL	NULL	0	NULL	chain	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	This effect is caused by a noncooperative interaction of water molecules with electrophilic groups of amino acid and by intramolecular hydrogen bond , allowing proton transfer from the carboxylic to the amine group , accomplishing by the chain of two to four water molecules .
	manualset3
185570	10	414329	7	NULL	NULL	0	NULL	 two water molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	This effect is caused by a noncooperative interaction of water molecules with electrophilic groups of amino acid and by intramolecular hydrogen bond , allowing proton transfer from the carboxylic to the amine group , accomplishing by the chain of two to four water molecules .
	manualset3
185571	11	414329	7	NULL	NULL	0	NULL	four water molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	This effect is caused by a noncooperative interaction of water molecules with electrophilic groups of amino acid and by intramolecular hydrogen bond , allowing proton transfer from the carboxylic to the amine group , accomplishing by the chain of two to four water molecules .
	manualset3
185572	12	414329	7	NULL	NULL	0	NULL	amine group	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This effect is caused by a noncooperative interaction of water molecules with electrophilic groups of amino acid and by intramolecular hydrogen bond , allowing proton transfer from the carboxylic to the amine group , accomplishing by the chain of two to four water molecules .
	manualset3
185573	1	414330	7	NULL	NULL	0	NULL	effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This effect is thought to be mediated by inhibition of tumor necrosis factor-alpha ( TNFalpha ) - mediated long-terminal repeat ( LTR ) - driven expression .
	manualset3
185574	2	414330	7	NULL	NULL	0	NULL	inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This effect is thought to be mediated by inhibition of tumor necrosis factor-alpha ( TNFalpha ) - mediated long-terminal repeat ( LTR ) - driven expression .
	manualset3
185575	3	414330	7	NULL	NULL	0	NULL	tumor necrosis factor-alpha ( TNFalpha ) - mediated long-terminal repeat ( LTR ) - driven expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This effect is thought to be mediated by inhibition of tumor necrosis factor-alpha ( TNFalpha ) - mediated long-terminal repeat ( LTR ) - driven expression .
	manualset3
185861	1	415331	7	NULL	NULL	0	NULL	demographic characteristics	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After accounting for demographic characteristics in logistic regression equations , findings suggested that interventions addressing symptom education , service continuity , and daily structure were most effective in preventing inpatient stay among individuals with four or more prior hospitalizations .
	manualset3
185862	2	415331	7	NULL	NULL	0	NULL	logistic regression equations	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	After accounting for demographic characteristics in logistic regression equations , findings suggested that interventions addressing symptom education , service continuity , and daily structure were most effective in preventing inpatient stay among individuals with four or more prior hospitalizations .
	manualset3
185863	3	415331	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After accounting for demographic characteristics in logistic regression equations , findings suggested that interventions addressing symptom education , service continuity , and daily structure were most effective in preventing inpatient stay among individuals with four or more prior hospitalizations .
	manualset3
185864	4	415331	7	NULL	NULL	0	NULL	interventions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After accounting for demographic characteristics in logistic regression equations , findings suggested that interventions addressing symptom education , service continuity , and daily structure were most effective in preventing inpatient stay among individuals with four or more prior hospitalizations .
	manualset3
185865	5	415331	7	NULL	NULL	NULL	NULL	 symptom education	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After accounting for demographic characteristics in logistic regression equations , findings suggested that interventions addressing symptom education , service continuity , and daily structure were most effective in preventing inpatient stay among individuals with four or more prior hospitalizations .
	manualset3
185866	6	415331	7	NULL	NULL	0	NULL	service continuity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After accounting for demographic characteristics in logistic regression equations , findings suggested that interventions addressing symptom education , service continuity , and daily structure were most effective in preventing inpatient stay among individuals with four or more prior hospitalizations .
	manualset3
185867	7	415331	7	NULL	NULL	0	NULL	daily structure 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After accounting for demographic characteristics in logistic regression equations , findings suggested that interventions addressing symptom education , service continuity , and daily structure were most effective in preventing inpatient stay among individuals with four or more prior hospitalizations .
	manualset3
185868	8	415331	7	NULL	NULL	0	NULL	inpatient stay	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After accounting for demographic characteristics in logistic regression equations , findings suggested that interventions addressing symptom education , service continuity , and daily structure were most effective in preventing inpatient stay among individuals with four or more prior hospitalizations .
	manualset3
185869	9	415331	7	NULL	NULL	0	NULL	individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	After accounting for demographic characteristics in logistic regression equations , findings suggested that interventions addressing symptom education , service continuity , and daily structure were most effective in preventing inpatient stay among individuals with four or more prior hospitalizations .
	manualset3
185870	10	415331	7	NULL	NULL	0	NULL	four	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After accounting for demographic characteristics in logistic regression equations , findings suggested that interventions addressing symptom education , service continuity , and daily structure were most effective in preventing inpatient stay among individuals with four or more prior hospitalizations .
	manualset3
185871	11	415331	7	NULL	NULL	0	NULL	hospitalizations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After accounting for demographic characteristics in logistic regression equations , findings suggested that interventions addressing symptom education , service continuity , and daily structure were most effective in preventing inpatient stay among individuals with four or more prior hospitalizations .
	manualset3
185872	1	415332	7	NULL	NULL	0	NULL	SOFFI Method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To be clear , the SOFFI Method is not focused on the amount of food taken in but on the conduct of the feeding and the development of competent infant feeding behavior that , consequently , assures the intake of food necessary for growth .
	manualset3
185873	2	415332	7	NULL	NULL	0	NULL	 amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To be clear , the SOFFI Method is not focused on the amount of food taken in but on the conduct of the feeding and the development of competent infant feeding behavior that , consequently , assures the intake of food necessary for growth .
	manualset3
185874	3	415332	7	NULL	NULL	0	NULL	food	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	To be clear , the SOFFI Method is not focused on the amount of food taken in but on the conduct of the feeding and the development of competent infant feeding behavior that , consequently , assures the intake of food necessary for growth .
	manualset3
185875	4	415332	7	NULL	NULL	0	NULL	conduct of the feeding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To be clear , the SOFFI Method is not focused on the amount of food taken in but on the conduct of the feeding and the development of competent infant feeding behavior that , consequently , assures the intake of food necessary for growth .
	manualset3
185876	5	415332	7	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To be clear , the SOFFI Method is not focused on the amount of food taken in but on the conduct of the feeding and the development of competent infant feeding behavior that , consequently , assures the intake of food necessary for growth .
	manualset3
185877	6	415332	7	NULL	NULL	0	NULL	competent infant feeding behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To be clear , the SOFFI Method is not focused on the amount of food taken in but on the conduct of the feeding and the development of competent infant feeding behavior that , consequently , assures the intake of food necessary for growth .
	manualset3
185878	7	415332	7	NULL	NULL	0	NULL	intake of food	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To be clear , the SOFFI Method is not focused on the amount of food taken in but on the conduct of the feeding and the development of competent infant feeding behavior that , consequently , assures the intake of food necessary for growth .
	manualset3
185879	8	415332	7	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To be clear , the SOFFI Method is not focused on the amount of food taken in but on the conduct of the feeding and the development of competent infant feeding behavior that , consequently , assures the intake of food necessary for growth .
	manualset3
185880	1	415333	7	NULL	NULL	0	NULL	antibody	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To be effective the antibody must bind to the fibrin component of the clot .
	manualset3
185881	2	415333	7	NULL	NULL	NULL	NULL	 fibrin component	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To be effective the antibody must bind to the fibrin component of the clot .
	manualset3
185882	3	415333	7	NULL	NULL	0	NULL	clot	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To be effective the antibody must bind to the fibrin component of the clot .
	manualset3
185883	1	415334	7	NULL	NULL	0	NULL	molecular basis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To begin identifying the molecular basis for gap junction channel behavior in the human heart , a tissue that expresses connexin43 , we used site-directed mutagenesis to generate mutant cDNAs of human connexin43 with shortened cytoplasmic tail domains .
	manualset3
185884	2	415334	7	NULL	NULL	0	NULL	gap junction channel behavior	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To begin identifying the molecular basis for gap junction channel behavior in the human heart , a tissue that expresses connexin43 , we used site-directed mutagenesis to generate mutant cDNAs of human connexin43 with shortened cytoplasmic tail domains .
	manualset3
185885	3	415334	7	NULL	NULL	0	NULL	 human heart	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To begin identifying the molecular basis for gap junction channel behavior in the human heart , a tissue that expresses connexin43 , we used site-directed mutagenesis to generate mutant cDNAs of human connexin43 with shortened cytoplasmic tail domains .
	manualset3
185886	4	415334	7	NULL	NULL	0	NULL	 tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	To begin identifying the molecular basis for gap junction channel behavior in the human heart , a tissue that expresses connexin43 , we used site-directed mutagenesis to generate mutant cDNAs of human connexin43 with shortened cytoplasmic tail domains .
	manualset3
185887	5	415334	7	NULL	NULL	0	NULL	connexin43	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To begin identifying the molecular basis for gap junction channel behavior in the human heart , a tissue that expresses connexin43 , we used site-directed mutagenesis to generate mutant cDNAs of human connexin43 with shortened cytoplasmic tail domains .
	manualset3
185888	6	415334	7	NULL	NULL	0	NULL	site-directed mutagenesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To begin identifying the molecular basis for gap junction channel behavior in the human heart , a tissue that expresses connexin43 , we used site-directed mutagenesis to generate mutant cDNAs of human connexin43 with shortened cytoplasmic tail domains .
	manualset3
185889	7	415334	7	NULL	NULL	0	NULL	mutant cDNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To begin identifying the molecular basis for gap junction channel behavior in the human heart , a tissue that expresses connexin43 , we used site-directed mutagenesis to generate mutant cDNAs of human connexin43 with shortened cytoplasmic tail domains .
	manualset3
185890	8	415334	7	NULL	NULL	0	NULL	human connexin43	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To begin identifying the molecular basis for gap junction channel behavior in the human heart , a tissue that expresses connexin43 , we used site-directed mutagenesis to generate mutant cDNAs of human connexin43 with shortened cytoplasmic tail domains .
	manualset3
185891	9	415334	7	NULL	NULL	0	NULL	shortened cytoplasmic tail domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	To begin identifying the molecular basis for gap junction channel behavior in the human heart , a tissue that expresses connexin43 , we used site-directed mutagenesis to generate mutant cDNAs of human connexin43 with shortened cytoplasmic tail domains .
	manualset3
185892	1	415335	7	NULL	NULL	0	NULL	 factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To better define the factors facilitating noncytolytic clearance of SINV in different regions of the central nervous system ( CNS ) and the roles of innate and adaptive immune responses at different times during infection , we have characterized SINV infection and clearance in the brain , brain stem , and spinal cords of severe combined immunodeficiency ( SCID ) and C57BL/6 ( wild-type ( WT ) ) mice and mice deficient in beta interferon ( IFN-beta ) ( BKO ) , antibody ( muMT ) , IFN-gamma ( GKO ) , IFN-gamma receptor ( GRKO ) , and both antibody and IFN-gamma ( muMT/GKO ) .
	manualset3
185893	2	415335	7	NULL	NULL	NULL	NULL	noncytolytic clearance	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To better define the factors facilitating noncytolytic clearance of SINV in different regions of the central nervous system ( CNS ) and the roles of innate and adaptive immune responses at different times during infection , we have characterized SINV infection and clearance in the brain , brain stem , and spinal cords of severe combined immunodeficiency ( SCID ) and C57BL/6 ( wild-type ( WT ) ) mice and mice deficient in beta interferon ( IFN-beta ) ( BKO ) , antibody ( muMT ) , IFN-gamma ( GKO ) , IFN-gamma receptor ( GRKO ) , and both antibody and IFN-gamma ( muMT/GKO ) .
	manualset3
185894	3	415335	7	NULL	NULL	0	NULL	SINV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To better define the factors facilitating noncytolytic clearance of SINV in different regions of the central nervous system ( CNS ) and the roles of innate and adaptive immune responses at different times during infection , we have characterized SINV infection and clearance in the brain , brain stem , and spinal cords of severe combined immunodeficiency ( SCID ) and C57BL/6 ( wild-type ( WT ) ) mice and mice deficient in beta interferon ( IFN-beta ) ( BKO ) , antibody ( muMT ) , IFN-gamma ( GKO ) , IFN-gamma receptor ( GRKO ) , and both antibody and IFN-gamma ( muMT/GKO ) .
	manualset3
185895	4	415335	7	NULL	NULL	0	NULL	 different regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To better define the factors facilitating noncytolytic clearance of SINV in different regions of the central nervous system ( CNS ) and the roles of innate and adaptive immune responses at different times during infection , we have characterized SINV infection and clearance in the brain , brain stem , and spinal cords of severe combined immunodeficiency ( SCID ) and C57BL/6 ( wild-type ( WT ) ) mice and mice deficient in beta interferon ( IFN-beta ) ( BKO ) , antibody ( muMT ) , IFN-gamma ( GKO ) , IFN-gamma receptor ( GRKO ) , and both antibody and IFN-gamma ( muMT/GKO ) .
	manualset3
185896	5	415335	7	NULL	NULL	0	NULL	 central nervous system ( CNS )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To better define the factors facilitating noncytolytic clearance of SINV in different regions of the central nervous system ( CNS ) and the roles of innate and adaptive immune responses at different times during infection , we have characterized SINV infection and clearance in the brain , brain stem , and spinal cords of severe combined immunodeficiency ( SCID ) and C57BL/6 ( wild-type ( WT ) ) mice and mice deficient in beta interferon ( IFN-beta ) ( BKO ) , antibody ( muMT ) , IFN-gamma ( GKO ) , IFN-gamma receptor ( GRKO ) , and both antibody and IFN-gamma ( muMT/GKO ) .
	manualset3
185897	6	415335	7	NULL	NULL	0	NULL	roles	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To better define the factors facilitating noncytolytic clearance of SINV in different regions of the central nervous system ( CNS ) and the roles of innate and adaptive immune responses at different times during infection , we have characterized SINV infection and clearance in the brain , brain stem , and spinal cords of severe combined immunodeficiency ( SCID ) and C57BL/6 ( wild-type ( WT ) ) mice and mice deficient in beta interferon ( IFN-beta ) ( BKO ) , antibody ( muMT ) , IFN-gamma ( GKO ) , IFN-gamma receptor ( GRKO ) , and both antibody and IFN-gamma ( muMT/GKO ) .
	manualset3
185898	7	415335	7	NULL	NULL	0	NULL	innate immune responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To better define the factors facilitating noncytolytic clearance of SINV in different regions of the central nervous system ( CNS ) and the roles of innate and adaptive immune responses at different times during infection , we have characterized SINV infection and clearance in the brain , brain stem , and spinal cords of severe combined immunodeficiency ( SCID ) and C57BL/6 ( wild-type ( WT ) ) mice and mice deficient in beta interferon ( IFN-beta ) ( BKO ) , antibody ( muMT ) , IFN-gamma ( GKO ) , IFN-gamma receptor ( GRKO ) , and both antibody and IFN-gamma ( muMT/GKO ) .
	manualset3
185899	8	415335	7	NULL	NULL	0	NULL	adaptive immune responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To better define the factors facilitating noncytolytic clearance of SINV in different regions of the central nervous system ( CNS ) and the roles of innate and adaptive immune responses at different times during infection , we have characterized SINV infection and clearance in the brain , brain stem , and spinal cords of severe combined immunodeficiency ( SCID ) and C57BL/6 ( wild-type ( WT ) ) mice and mice deficient in beta interferon ( IFN-beta ) ( BKO ) , antibody ( muMT ) , IFN-gamma ( GKO ) , IFN-gamma receptor ( GRKO ) , and both antibody and IFN-gamma ( muMT/GKO ) .
	manualset3
185900	9	415335	7	NULL	NULL	0	NULL	 times	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	To better define the factors facilitating noncytolytic clearance of SINV in different regions of the central nervous system ( CNS ) and the roles of innate and adaptive immune responses at different times during infection , we have characterized SINV infection and clearance in the brain , brain stem , and spinal cords of severe combined immunodeficiency ( SCID ) and C57BL/6 ( wild-type ( WT ) ) mice and mice deficient in beta interferon ( IFN-beta ) ( BKO ) , antibody ( muMT ) , IFN-gamma ( GKO ) , IFN-gamma receptor ( GRKO ) , and both antibody and IFN-gamma ( muMT/GKO ) .
	manualset3
185901	10	415335	7	NULL	NULL	0	NULL	infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To better define the factors facilitating noncytolytic clearance of SINV in different regions of the central nervous system ( CNS ) and the roles of innate and adaptive immune responses at different times during infection , we have characterized SINV infection and clearance in the brain , brain stem , and spinal cords of severe combined immunodeficiency ( SCID ) and C57BL/6 ( wild-type ( WT ) ) mice and mice deficient in beta interferon ( IFN-beta ) ( BKO ) , antibody ( muMT ) , IFN-gamma ( GKO ) , IFN-gamma receptor ( GRKO ) , and both antibody and IFN-gamma ( muMT/GKO ) .
	manualset3
185902	11	415335	7	NULL	NULL	0	NULL	SINV infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To better define the factors facilitating noncytolytic clearance of SINV in different regions of the central nervous system ( CNS ) and the roles of innate and adaptive immune responses at different times during infection , we have characterized SINV infection and clearance in the brain , brain stem , and spinal cords of severe combined immunodeficiency ( SCID ) and C57BL/6 ( wild-type ( WT ) ) mice and mice deficient in beta interferon ( IFN-beta ) ( BKO ) , antibody ( muMT ) , IFN-gamma ( GKO ) , IFN-gamma receptor ( GRKO ) , and both antibody and IFN-gamma ( muMT/GKO ) .
	manualset3
185903	12	415335	7	NULL	NULL	0	NULL	clearance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To better define the factors facilitating noncytolytic clearance of SINV in different regions of the central nervous system ( CNS ) and the roles of innate and adaptive immune responses at different times during infection , we have characterized SINV infection and clearance in the brain , brain stem , and spinal cords of severe combined immunodeficiency ( SCID ) and C57BL/6 ( wild-type ( WT ) ) mice and mice deficient in beta interferon ( IFN-beta ) ( BKO ) , antibody ( muMT ) , IFN-gamma ( GKO ) , IFN-gamma receptor ( GRKO ) , and both antibody and IFN-gamma ( muMT/GKO ) .
	manualset3
185904	13	415335	7	NULL	NULL	0	NULL	brain 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To better define the factors facilitating noncytolytic clearance of SINV in different regions of the central nervous system ( CNS ) and the roles of innate and adaptive immune responses at different times during infection , we have characterized SINV infection and clearance in the brain , brain stem , and spinal cords of severe combined immunodeficiency ( SCID ) and C57BL/6 ( wild-type ( WT ) ) mice and mice deficient in beta interferon ( IFN-beta ) ( BKO ) , antibody ( muMT ) , IFN-gamma ( GKO ) , IFN-gamma receptor ( GRKO ) , and both antibody and IFN-gamma ( muMT/GKO ) .
	manualset3
185905	14	415335	7	NULL	NULL	0	NULL	brain stem	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To better define the factors facilitating noncytolytic clearance of SINV in different regions of the central nervous system ( CNS ) and the roles of innate and adaptive immune responses at different times during infection , we have characterized SINV infection and clearance in the brain , brain stem , and spinal cords of severe combined immunodeficiency ( SCID ) and C57BL/6 ( wild-type ( WT ) ) mice and mice deficient in beta interferon ( IFN-beta ) ( BKO ) , antibody ( muMT ) , IFN-gamma ( GKO ) , IFN-gamma receptor ( GRKO ) , and both antibody and IFN-gamma ( muMT/GKO ) .
	manualset3
185906	15	415335	7	NULL	NULL	0	NULL	 spinal cords	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To better define the factors facilitating noncytolytic clearance of SINV in different regions of the central nervous system ( CNS ) and the roles of innate and adaptive immune responses at different times during infection , we have characterized SINV infection and clearance in the brain , brain stem , and spinal cords of severe combined immunodeficiency ( SCID ) and C57BL/6 ( wild-type ( WT ) ) mice and mice deficient in beta interferon ( IFN-beta ) ( BKO ) , antibody ( muMT ) , IFN-gamma ( GKO ) , IFN-gamma receptor ( GRKO ) , and both antibody and IFN-gamma ( muMT/GKO ) .
	manualset3
185907	16	415335	7	NULL	NULL	0	NULL	severe combined immunodeficiency ( SCID )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To better define the factors facilitating noncytolytic clearance of SINV in different regions of the central nervous system ( CNS ) and the roles of innate and adaptive immune responses at different times during infection , we have characterized SINV infection and clearance in the brain , brain stem , and spinal cords of severe combined immunodeficiency ( SCID ) and C57BL/6 ( wild-type ( WT ) ) mice and mice deficient in beta interferon ( IFN-beta ) ( BKO ) , antibody ( muMT ) , IFN-gamma ( GKO ) , IFN-gamma receptor ( GRKO ) , and both antibody and IFN-gamma ( muMT/GKO ) .
	manualset3
185908	17	415335	7	NULL	NULL	0	NULL	C57BL/6 ( wild-type ( WT ) ) mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To better define the factors facilitating noncytolytic clearance of SINV in different regions of the central nervous system ( CNS ) and the roles of innate and adaptive immune responses at different times during infection , we have characterized SINV infection and clearance in the brain , brain stem , and spinal cords of severe combined immunodeficiency ( SCID ) and C57BL/6 ( wild-type ( WT ) ) mice and mice deficient in beta interferon ( IFN-beta ) ( BKO ) , antibody ( muMT ) , IFN-gamma ( GKO ) , IFN-gamma receptor ( GRKO ) , and both antibody and IFN-gamma ( muMT/GKO ) .
	manualset3
185909	18	415335	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To better define the factors facilitating noncytolytic clearance of SINV in different regions of the central nervous system ( CNS ) and the roles of innate and adaptive immune responses at different times during infection , we have characterized SINV infection and clearance in the brain , brain stem , and spinal cords of severe combined immunodeficiency ( SCID ) and C57BL/6 ( wild-type ( WT ) ) mice and mice deficient in beta interferon ( IFN-beta ) ( BKO ) , antibody ( muMT ) , IFN-gamma ( GKO ) , IFN-gamma receptor ( GRKO ) , and both antibody and IFN-gamma ( muMT/GKO ) .
	manualset3
185910	19	415335	7	NULL	NULL	NULL	NULL	beta interferon ( IFN-beta) ( BKO )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To better define the factors facilitating noncytolytic clearance of SINV in different regions of the central nervous system ( CNS ) and the roles of innate and adaptive immune responses at different times during infection , we have characterized SINV infection and clearance in the brain , brain stem , and spinal cords of severe combined immunodeficiency ( SCID ) and C57BL/6 ( wild-type ( WT ) ) mice and mice deficient in beta interferon ( IFN-beta ) ( BKO ) , antibody ( muMT ) , IFN-gamma ( GKO ) , IFN-gamma receptor ( GRKO ) , and both antibody and IFN-gamma ( muMT/GKO ) .
	manualset3
185911	20	415335	7	NULL	NULL	0	NULL	antibody ( muMT )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To better define the factors facilitating noncytolytic clearance of SINV in different regions of the central nervous system ( CNS ) and the roles of innate and adaptive immune responses at different times during infection , we have characterized SINV infection and clearance in the brain , brain stem , and spinal cords of severe combined immunodeficiency ( SCID ) and C57BL/6 ( wild-type ( WT ) ) mice and mice deficient in beta interferon ( IFN-beta ) ( BKO ) , antibody ( muMT ) , IFN-gamma ( GKO ) , IFN-gamma receptor ( GRKO ) , and both antibody and IFN-gamma ( muMT/GKO ) .
	manualset3
185912	21	415335	7	NULL	NULL	0	NULL	IFN-gamma ( GKO )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To better define the factors facilitating noncytolytic clearance of SINV in different regions of the central nervous system ( CNS ) and the roles of innate and adaptive immune responses at different times during infection , we have characterized SINV infection and clearance in the brain , brain stem , and spinal cords of severe combined immunodeficiency ( SCID ) and C57BL/6 ( wild-type ( WT ) ) mice and mice deficient in beta interferon ( IFN-beta ) ( BKO ) , antibody ( muMT ) , IFN-gamma ( GKO ) , IFN-gamma receptor ( GRKO ) , and both antibody and IFN-gamma ( muMT/GKO ) .
	manualset3
185913	22	415335	7	NULL	NULL	0	NULL	IFN-gamma receptor ( GRKO )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To better define the factors facilitating noncytolytic clearance of SINV in different regions of the central nervous system ( CNS ) and the roles of innate and adaptive immune responses at different times during infection , we have characterized SINV infection and clearance in the brain , brain stem , and spinal cords of severe combined immunodeficiency ( SCID ) and C57BL/6 ( wild-type ( WT ) ) mice and mice deficient in beta interferon ( IFN-beta ) ( BKO ) , antibody ( muMT ) , IFN-gamma ( GKO ) , IFN-gamma receptor ( GRKO ) , and both antibody and IFN-gamma ( muMT/GKO ) .
	manualset3
185914	23	415335	7	NULL	NULL	0	NULL	 antibody 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To better define the factors facilitating noncytolytic clearance of SINV in different regions of the central nervous system ( CNS ) and the roles of innate and adaptive immune responses at different times during infection , we have characterized SINV infection and clearance in the brain , brain stem , and spinal cords of severe combined immunodeficiency ( SCID ) and C57BL/6 ( wild-type ( WT ) ) mice and mice deficient in beta interferon ( IFN-beta ) ( BKO ) , antibody ( muMT ) , IFN-gamma ( GKO ) , IFN-gamma receptor ( GRKO ) , and both antibody and IFN-gamma ( muMT/GKO ) .
	manualset3
185915	24	415335	7	NULL	NULL	0	NULL	IFN-gamma ( muMT/GKO )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To better define the factors facilitating noncytolytic clearance of SINV in different regions of the central nervous system ( CNS ) and the roles of innate and adaptive immune responses at different times during infection , we have characterized SINV infection and clearance in the brain , brain stem , and spinal cords of severe combined immunodeficiency ( SCID ) and C57BL/6 ( wild-type ( WT ) ) mice and mice deficient in beta interferon ( IFN-beta ) ( BKO ) , antibody ( muMT ) , IFN-gamma ( GKO ) , IFN-gamma receptor ( GRKO ) , and both antibody and IFN-gamma ( muMT/GKO ) .
	manualset3
185916	1	415336	7	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand such differences , we assessed skeletal muscle histomorphological and energetic characteristics in 10 control HbAA subjects ( C ) , 5 subjects with alpha-t ( alpha-t ) , 6 SCT carriers ( SCT ) and 9 SCT carriers with alpha-t ( SCT/alpha-t ) .
	manualset3
185917	2	415336	7	NULL	NULL	0	NULL	skeletal muscle histomorphological characteristics	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand such differences , we assessed skeletal muscle histomorphological and energetic characteristics in 10 control HbAA subjects ( C ) , 5 subjects with alpha-t ( alpha-t ) , 6 SCT carriers ( SCT ) and 9 SCT carriers with alpha-t ( SCT/alpha-t ) .
	manualset3
185918	3	415336	7	NULL	NULL	0	NULL	energetic characteristics	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand such differences , we assessed skeletal muscle histomorphological and energetic characteristics in 10 control HbAA subjects ( C ) , 5 subjects with alpha-t ( alpha-t ) , 6 SCT carriers ( SCT ) and 9 SCT carriers with alpha-t ( SCT/alpha-t ) .
	manualset3
185919	4	415336	7	NULL	NULL	NULL	NULL	10 control HbAA subjects ( C )	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To better understand such differences , we assessed skeletal muscle histomorphological and energetic characteristics in 10 control HbAA subjects ( C ) , 5 subjects with alpha-t ( alpha-t ) , 6 SCT carriers ( SCT ) and 9 SCT carriers with alpha-t ( SCT/alpha-t ) .
	manualset3
185920	5	415336	7	NULL	NULL	NULL	NULL	5 subjects with alpha-t ( alpha-t )	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To better understand such differences , we assessed skeletal muscle histomorphological and energetic characteristics in 10 control HbAA subjects ( C ) , 5 subjects with alpha-t ( alpha-t ) , 6 SCT carriers ( SCT ) and 9 SCT carriers with alpha-t ( SCT/alpha-t ) .
	manualset3
185921	6	415336	7	NULL	NULL	NULL	NULL	6 SCT carriers ( SCT )	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To better understand such differences , we assessed skeletal muscle histomorphological and energetic characteristics in 10 control HbAA subjects ( C ) , 5 subjects with alpha-t ( alpha-t ) , 6 SCT carriers ( SCT ) and 9 SCT carriers with alpha-t ( SCT/alpha-t ) .
	manualset3
185922	7	415336	7	NULL	NULL	NULL	NULL	9 SCT carriers with alpha-t ( SCT/alpha-t )	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To better understand such differences , we assessed skeletal muscle histomorphological and energetic characteristics in 10 control HbAA subjects ( C ) , 5 subjects with alpha-t ( alpha-t ) , 6 SCT carriers ( SCT ) and 9 SCT carriers with alpha-t ( SCT/alpha-t ) .
	manualset3
185928	1	415337	7	NULL	NULL	0	NULL	challenges 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the challenges associated with the CVD synthesis of the ternary chalcogenide , computational fluid dynamics simulations are performed to quantify 3D thermal and momentum transients in the growth conditions .
	manualset3
185929	2	415337	7	NULL	NULL	0	NULL	CVD synthesis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the challenges associated with the CVD synthesis of the ternary chalcogenide , computational fluid dynamics simulations are performed to quantify 3D thermal and momentum transients in the growth conditions .
	manualset3
185930	3	415337	7	NULL	NULL	0	NULL	ternary chalcogenide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the challenges associated with the CVD synthesis of the ternary chalcogenide , computational fluid dynamics simulations are performed to quantify 3D thermal and momentum transients in the growth conditions .
	manualset3
185931	4	415337	7	NULL	NULL	0	NULL	computational fluid dynamics simulations	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the challenges associated with the CVD synthesis of the ternary chalcogenide , computational fluid dynamics simulations are performed to quantify 3D thermal and momentum transients in the growth conditions .
	manualset3
185932	5	415337	7	NULL	NULL	NULL	NULL	3D thermal transients	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To better understand the challenges associated with the CVD synthesis of the ternary chalcogenide , computational fluid dynamics simulations are performed to quantify 3D thermal and momentum transients in the growth conditions .
	manualset3
185933	6	415337	7	NULL	NULL	0	NULL	momentum transients	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the challenges associated with the CVD synthesis of the ternary chalcogenide , computational fluid dynamics simulations are performed to quantify 3D thermal and momentum transients in the growth conditions .
	manualset3
185934	7	415337	7	NULL	NULL	0	NULL	growth conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the challenges associated with the CVD synthesis of the ternary chalcogenide , computational fluid dynamics simulations are performed to quantify 3D thermal and momentum transients in the growth conditions .
	manualset3
185937	1	415338	7	NULL	NULL	0	NULL	evolution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the evolution of red-green color vision in vertebrates , we inferred the amino acid sequences of the ancestral pigments of 11 selected visual pigments : the LWS pigments of cave fish ( Astyanax fasciatus ) , frog ( Xenopus laevis ) , chicken ( Gallus gallus ) , chameleon ( Anolis carolinensis ) , goat ( Capra hircus ) , and human ( Homo sapiens ) ; and the MWS pigments of cave fish , gecko ( Gekko gekko ) , mouse ( Mus musculus ) , squirrel ( Sciurus carolinensis ) , and human .
	manualset3
185943	2	415338	7	NULL	NULL	0	NULL	red-green color vision	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the evolution of red-green color vision in vertebrates , we inferred the amino acid sequences of the ancestral pigments of 11 selected visual pigments : the LWS pigments of cave fish ( Astyanax fasciatus ) , frog ( Xenopus laevis ) , chicken ( Gallus gallus ) , chameleon ( Anolis carolinensis ) , goat ( Capra hircus ) , and human ( Homo sapiens ) ; and the MWS pigments of cave fish , gecko ( Gekko gekko ) , mouse ( Mus musculus ) , squirrel ( Sciurus carolinensis ) , and human .
	manualset3
185945	3	415338	7	NULL	NULL	0	NULL	 vertebrates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the evolution of red-green color vision in vertebrates , we inferred the amino acid sequences of the ancestral pigments of 11 selected visual pigments : the LWS pigments of cave fish ( Astyanax fasciatus ) , frog ( Xenopus laevis ) , chicken ( Gallus gallus ) , chameleon ( Anolis carolinensis ) , goat ( Capra hircus ) , and human ( Homo sapiens ) ; and the MWS pigments of cave fish , gecko ( Gekko gekko ) , mouse ( Mus musculus ) , squirrel ( Sciurus carolinensis ) , and human .
	manualset3
185946	4	415338	7	NULL	NULL	0	NULL	amino acid sequences	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the evolution of red-green color vision in vertebrates , we inferred the amino acid sequences of the ancestral pigments of 11 selected visual pigments : the LWS pigments of cave fish ( Astyanax fasciatus ) , frog ( Xenopus laevis ) , chicken ( Gallus gallus ) , chameleon ( Anolis carolinensis ) , goat ( Capra hircus ) , and human ( Homo sapiens ) ; and the MWS pigments of cave fish , gecko ( Gekko gekko ) , mouse ( Mus musculus ) , squirrel ( Sciurus carolinensis ) , and human .
	manualset3
185948	5	415338	7	NULL	NULL	NULL	NULL	ancestral pigments 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To better understand the evolution of red-green color vision in vertebrates , we inferred the amino acid sequences of the ancestral pigments of 11 selected visual pigments : the LWS pigments of cave fish ( Astyanax fasciatus ) , frog ( Xenopus laevis ) , chicken ( Gallus gallus ) , chameleon ( Anolis carolinensis ) , goat ( Capra hircus ) , and human ( Homo sapiens ) ; and the MWS pigments of cave fish , gecko ( Gekko gekko ) , mouse ( Mus musculus ) , squirrel ( Sciurus carolinensis ) , and human .
	manualset3
185950	6	415338	7	NULL	NULL	0	NULL	11 selected visual pigments 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the evolution of red-green color vision in vertebrates , we inferred the amino acid sequences of the ancestral pigments of 11 selected visual pigments : the LWS pigments of cave fish ( Astyanax fasciatus ) , frog ( Xenopus laevis ) , chicken ( Gallus gallus ) , chameleon ( Anolis carolinensis ) , goat ( Capra hircus ) , and human ( Homo sapiens ) ; and the MWS pigments of cave fish , gecko ( Gekko gekko ) , mouse ( Mus musculus ) , squirrel ( Sciurus carolinensis ) , and human .
	manualset3
185952	7	415338	7	NULL	NULL	0	NULL	LWS pigments	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the evolution of red-green color vision in vertebrates , we inferred the amino acid sequences of the ancestral pigments of 11 selected visual pigments : the LWS pigments of cave fish ( Astyanax fasciatus ) , frog ( Xenopus laevis ) , chicken ( Gallus gallus ) , chameleon ( Anolis carolinensis ) , goat ( Capra hircus ) , and human ( Homo sapiens ) ; and the MWS pigments of cave fish , gecko ( Gekko gekko ) , mouse ( Mus musculus ) , squirrel ( Sciurus carolinensis ) , and human .
	manualset3
185957	8	415338	7	NULL	NULL	0	NULL	cave fish ( Astyanax fasciatus )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the evolution of red-green color vision in vertebrates , we inferred the amino acid sequences of the ancestral pigments of 11 selected visual pigments : the LWS pigments of cave fish ( Astyanax fasciatus ) , frog ( Xenopus laevis ) , chicken ( Gallus gallus ) , chameleon ( Anolis carolinensis ) , goat ( Capra hircus ) , and human ( Homo sapiens ) ; and the MWS pigments of cave fish , gecko ( Gekko gekko ) , mouse ( Mus musculus ) , squirrel ( Sciurus carolinensis ) , and human .
	manualset3
185959	9	415338	7	NULL	NULL	0	NULL	frog ( Xenopus laevis )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the evolution of red-green color vision in vertebrates , we inferred the amino acid sequences of the ancestral pigments of 11 selected visual pigments : the LWS pigments of cave fish ( Astyanax fasciatus ) , frog ( Xenopus laevis ) , chicken ( Gallus gallus ) , chameleon ( Anolis carolinensis ) , goat ( Capra hircus ) , and human ( Homo sapiens ) ; and the MWS pigments of cave fish , gecko ( Gekko gekko ) , mouse ( Mus musculus ) , squirrel ( Sciurus carolinensis ) , and human .
	manualset3
185960	10	415338	7	NULL	NULL	0	NULL	chicken ( Gallus gallus )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the evolution of red-green color vision in vertebrates , we inferred the amino acid sequences of the ancestral pigments of 11 selected visual pigments : the LWS pigments of cave fish ( Astyanax fasciatus ) , frog ( Xenopus laevis ) , chicken ( Gallus gallus ) , chameleon ( Anolis carolinensis ) , goat ( Capra hircus ) , and human ( Homo sapiens ) ; and the MWS pigments of cave fish , gecko ( Gekko gekko ) , mouse ( Mus musculus ) , squirrel ( Sciurus carolinensis ) , and human .
	manualset3
185962	11	415338	7	NULL	NULL	0	NULL	chameleon ( Anolis carolinensis )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the evolution of red-green color vision in vertebrates , we inferred the amino acid sequences of the ancestral pigments of 11 selected visual pigments : the LWS pigments of cave fish ( Astyanax fasciatus ) , frog ( Xenopus laevis ) , chicken ( Gallus gallus ) , chameleon ( Anolis carolinensis ) , goat ( Capra hircus ) , and human ( Homo sapiens ) ; and the MWS pigments of cave fish , gecko ( Gekko gekko ) , mouse ( Mus musculus ) , squirrel ( Sciurus carolinensis ) , and human .
	manualset3
185963	12	415338	7	NULL	NULL	0	NULL	goat ( Capra hircus )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the evolution of red-green color vision in vertebrates , we inferred the amino acid sequences of the ancestral pigments of 11 selected visual pigments : the LWS pigments of cave fish ( Astyanax fasciatus ) , frog ( Xenopus laevis ) , chicken ( Gallus gallus ) , chameleon ( Anolis carolinensis ) , goat ( Capra hircus ) , and human ( Homo sapiens ) ; and the MWS pigments of cave fish , gecko ( Gekko gekko ) , mouse ( Mus musculus ) , squirrel ( Sciurus carolinensis ) , and human .
	manualset3
185965	13	415338	7	NULL	NULL	0	NULL	human ( Homo sapiens )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the evolution of red-green color vision in vertebrates , we inferred the amino acid sequences of the ancestral pigments of 11 selected visual pigments : the LWS pigments of cave fish ( Astyanax fasciatus ) , frog ( Xenopus laevis ) , chicken ( Gallus gallus ) , chameleon ( Anolis carolinensis ) , goat ( Capra hircus ) , and human ( Homo sapiens ) ; and the MWS pigments of cave fish , gecko ( Gekko gekko ) , mouse ( Mus musculus ) , squirrel ( Sciurus carolinensis ) , and human .
	manualset3
185967	14	415338	7	NULL	NULL	0	NULL	MWS pigments	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the evolution of red-green color vision in vertebrates , we inferred the amino acid sequences of the ancestral pigments of 11 selected visual pigments : the LWS pigments of cave fish ( Astyanax fasciatus ) , frog ( Xenopus laevis ) , chicken ( Gallus gallus ) , chameleon ( Anolis carolinensis ) , goat ( Capra hircus ) , and human ( Homo sapiens ) ; and the MWS pigments of cave fish , gecko ( Gekko gekko ) , mouse ( Mus musculus ) , squirrel ( Sciurus carolinensis ) , and human .
	manualset3
185969	15	415338	7	NULL	NULL	0	NULL	cave fish	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the evolution of red-green color vision in vertebrates , we inferred the amino acid sequences of the ancestral pigments of 11 selected visual pigments : the LWS pigments of cave fish ( Astyanax fasciatus ) , frog ( Xenopus laevis ) , chicken ( Gallus gallus ) , chameleon ( Anolis carolinensis ) , goat ( Capra hircus ) , and human ( Homo sapiens ) ; and the MWS pigments of cave fish , gecko ( Gekko gekko ) , mouse ( Mus musculus ) , squirrel ( Sciurus carolinensis ) , and human .
	manualset3
185970	16	415338	7	NULL	NULL	0	NULL	gecko ( Gekko gekko )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the evolution of red-green color vision in vertebrates , we inferred the amino acid sequences of the ancestral pigments of 11 selected visual pigments : the LWS pigments of cave fish ( Astyanax fasciatus ) , frog ( Xenopus laevis ) , chicken ( Gallus gallus ) , chameleon ( Anolis carolinensis ) , goat ( Capra hircus ) , and human ( Homo sapiens ) ; and the MWS pigments of cave fish , gecko ( Gekko gekko ) , mouse ( Mus musculus ) , squirrel ( Sciurus carolinensis ) , and human .
	manualset3
185971	17	415338	7	NULL	NULL	0	NULL	mouse ( Mus musculus )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the evolution of red-green color vision in vertebrates , we inferred the amino acid sequences of the ancestral pigments of 11 selected visual pigments : the LWS pigments of cave fish ( Astyanax fasciatus ) , frog ( Xenopus laevis ) , chicken ( Gallus gallus ) , chameleon ( Anolis carolinensis ) , goat ( Capra hircus ) , and human ( Homo sapiens ) ; and the MWS pigments of cave fish , gecko ( Gekko gekko ) , mouse ( Mus musculus ) , squirrel ( Sciurus carolinensis ) , and human .
	manualset3
185972	18	415338	7	NULL	NULL	0	NULL	squirrel ( Sciurus carolinensis )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the evolution of red-green color vision in vertebrates , we inferred the amino acid sequences of the ancestral pigments of 11 selected visual pigments : the LWS pigments of cave fish ( Astyanax fasciatus ) , frog ( Xenopus laevis ) , chicken ( Gallus gallus ) , chameleon ( Anolis carolinensis ) , goat ( Capra hircus ) , and human ( Homo sapiens ) ; and the MWS pigments of cave fish , gecko ( Gekko gekko ) , mouse ( Mus musculus ) , squirrel ( Sciurus carolinensis ) , and human .
	manualset3
185973	19	415338	7	NULL	NULL	0	NULL	human	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the evolution of red-green color vision in vertebrates , we inferred the amino acid sequences of the ancestral pigments of 11 selected visual pigments : the LWS pigments of cave fish ( Astyanax fasciatus ) , frog ( Xenopus laevis ) , chicken ( Gallus gallus ) , chameleon ( Anolis carolinensis ) , goat ( Capra hircus ) , and human ( Homo sapiens ) ; and the MWS pigments of cave fish , gecko ( Gekko gekko ) , mouse ( Mus musculus ) , squirrel ( Sciurus carolinensis ) , and human .
	manualset3
185976	1	415339	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the relationship between these two disorders and the role of collagen table thickening in the pathogenesis of diarrhea , colonic mucosal biopsy specimens from 24 patients with microscopic or collagenous colitis and 9 control subjects were analyzed using a computer-assisted morphometric method to evaluate the average thickness of the subepithelial collagen table .
	manualset3
185977	2	415339	7	NULL	NULL	0	NULL	two disorders 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the relationship between these two disorders and the role of collagen table thickening in the pathogenesis of diarrhea , colonic mucosal biopsy specimens from 24 patients with microscopic or collagenous colitis and 9 control subjects were analyzed using a computer-assisted morphometric method to evaluate the average thickness of the subepithelial collagen table .
	manualset3
185978	3	415339	7	NULL	NULL	0	NULL	 role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the relationship between these two disorders and the role of collagen table thickening in the pathogenesis of diarrhea , colonic mucosal biopsy specimens from 24 patients with microscopic or collagenous colitis and 9 control subjects were analyzed using a computer-assisted morphometric method to evaluate the average thickness of the subepithelial collagen table .
	manualset3
185979	4	415339	7	NULL	NULL	0	NULL	collagen table thickening 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the relationship between these two disorders and the role of collagen table thickening in the pathogenesis of diarrhea , colonic mucosal biopsy specimens from 24 patients with microscopic or collagenous colitis and 9 control subjects were analyzed using a computer-assisted morphometric method to evaluate the average thickness of the subepithelial collagen table .
	manualset3
185981	5	415339	7	NULL	NULL	0	NULL	pathogenesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the relationship between these two disorders and the role of collagen table thickening in the pathogenesis of diarrhea , colonic mucosal biopsy specimens from 24 patients with microscopic or collagenous colitis and 9 control subjects were analyzed using a computer-assisted morphometric method to evaluate the average thickness of the subepithelial collagen table .
	manualset3
185982	6	415339	7	NULL	NULL	0	NULL	diarrhea	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the relationship between these two disorders and the role of collagen table thickening in the pathogenesis of diarrhea , colonic mucosal biopsy specimens from 24 patients with microscopic or collagenous colitis and 9 control subjects were analyzed using a computer-assisted morphometric method to evaluate the average thickness of the subepithelial collagen table .
	manualset3
185991	7	415339	7	NULL	NULL	0	NULL	colonic mucosal biopsy specimens	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the relationship between these two disorders and the role of collagen table thickening in the pathogenesis of diarrhea , colonic mucosal biopsy specimens from 24 patients with microscopic or collagenous colitis and 9 control subjects were analyzed using a computer-assisted morphometric method to evaluate the average thickness of the subepithelial collagen table .
	manualset3
185992	8	415339	7	NULL	NULL	0	NULL	24 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the relationship between these two disorders and the role of collagen table thickening in the pathogenesis of diarrhea , colonic mucosal biopsy specimens from 24 patients with microscopic or collagenous colitis and 9 control subjects were analyzed using a computer-assisted morphometric method to evaluate the average thickness of the subepithelial collagen table .
	manualset3
185994	9	415339	7	NULL	NULL	0	NULL	microscopic colitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the relationship between these two disorders and the role of collagen table thickening in the pathogenesis of diarrhea , colonic mucosal biopsy specimens from 24 patients with microscopic or collagenous colitis and 9 control subjects were analyzed using a computer-assisted morphometric method to evaluate the average thickness of the subepithelial collagen table .
	manualset3
185996	10	415339	7	NULL	NULL	0	NULL	collagenous colitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the relationship between these two disorders and the role of collagen table thickening in the pathogenesis of diarrhea , colonic mucosal biopsy specimens from 24 patients with microscopic or collagenous colitis and 9 control subjects were analyzed using a computer-assisted morphometric method to evaluate the average thickness of the subepithelial collagen table .
	manualset3
185998	11	415339	7	NULL	NULL	0	NULL	9 control subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the relationship between these two disorders and the role of collagen table thickening in the pathogenesis of diarrhea , colonic mucosal biopsy specimens from 24 patients with microscopic or collagenous colitis and 9 control subjects were analyzed using a computer-assisted morphometric method to evaluate the average thickness of the subepithelial collagen table .
	manualset3
186000	12	415339	7	NULL	NULL	0	NULL	computer-assisted morphometric method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the relationship between these two disorders and the role of collagen table thickening in the pathogenesis of diarrhea , colonic mucosal biopsy specimens from 24 patients with microscopic or collagenous colitis and 9 control subjects were analyzed using a computer-assisted morphometric method to evaluate the average thickness of the subepithelial collagen table .
	manualset3
186004	13	415339	7	NULL	NULL	0	NULL	average thickness	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the relationship between these two disorders and the role of collagen table thickening in the pathogenesis of diarrhea , colonic mucosal biopsy specimens from 24 patients with microscopic or collagenous colitis and 9 control subjects were analyzed using a computer-assisted morphometric method to evaluate the average thickness of the subepithelial collagen table .
	manualset3
186005	14	415339	7	NULL	NULL	0	NULL	subepithelial collagen table 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the relationship between these two disorders and the role of collagen table thickening in the pathogenesis of diarrhea , colonic mucosal biopsy specimens from 24 patients with microscopic or collagenous colitis and 9 control subjects were analyzed using a computer-assisted morphometric method to evaluate the average thickness of the subepithelial collagen table .
	manualset3
186016	1	415340	7	NULL	NULL	NULL	NULL	understand	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To better understand the role of cytokines in seizures and their sequelae , we have characterized cytokine expression in an animal model of epilepsy .
	manualset3
186017	2	415340	7	NULL	NULL	0	NULL	 role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the role of cytokines in seizures and their sequelae , we have characterized cytokine expression in an animal model of epilepsy .
	manualset3
186018	3	415340	7	NULL	NULL	0	NULL	cytokines	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the role of cytokines in seizures and their sequelae , we have characterized cytokine expression in an animal model of epilepsy .
	manualset3
186019	4	415340	7	NULL	NULL	0	NULL	 seizures	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the role of cytokines in seizures and their sequelae , we have characterized cytokine expression in an animal model of epilepsy .
	manualset3
186020	5	415340	7	NULL	NULL	0	NULL	sequelae	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the role of cytokines in seizures and their sequelae , we have characterized cytokine expression in an animal model of epilepsy .
	manualset3
186021	6	415340	7	NULL	NULL	0	NULL	cytokine expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the role of cytokines in seizures and their sequelae , we have characterized cytokine expression in an animal model of epilepsy .
	manualset3
186023	7	415340	7	NULL	NULL	0	NULL	animal model	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the role of cytokines in seizures and their sequelae , we have characterized cytokine expression in an animal model of epilepsy .
	manualset3
186025	8	415340	7	NULL	NULL	0	NULL	epilepsy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To better understand the role of cytokines in seizures and their sequelae , we have characterized cytokine expression in an animal model of epilepsy .
	manualset3
186026	1	415341	7	NULL	NULL	0	NULL	buffer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After adding a buffer with low sugar concentration ( 10 mM glucoside ) a large amount of apolipoprotein H was recovered .
	manualset3
186027	2	415341	7	NULL	NULL	0	NULL	low sugar concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After adding a buffer with low sugar concentration ( 10 mM glucoside ) a large amount of apolipoprotein H was recovered .
	manualset3
186028	3	415341	7	NULL	NULL	0	NULL	10 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	After adding a buffer with low sugar concentration ( 10 mM glucoside ) a large amount of apolipoprotein H was recovered .
	manualset3
186029	4	415341	7	NULL	NULL	0	NULL	glucoside	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After adding a buffer with low sugar concentration ( 10 mM glucoside ) a large amount of apolipoprotein H was recovered .
	manualset3
186030	5	415341	7	NULL	NULL	0	NULL	amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After adding a buffer with low sugar concentration ( 10 mM glucoside ) a large amount of apolipoprotein H was recovered .
	manualset3
186031	6	415341	7	NULL	NULL	0	NULL	apolipoprotein H	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After adding a buffer with low sugar concentration ( 10 mM glucoside ) a large amount of apolipoprotein H was recovered .
	manualset3
186034	1	415342	7	NULL	NULL	0	NULL	To bundle or not to bundle	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	To bundle or not to bundle : lawmakers explore the question .
	manualset3
186036	2	415342	7	NULL	NULL	0	NULL	 lawmakers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To bundle or not to bundle : lawmakers explore the question .
	manualset3
186037	3	415342	7	NULL	NULL	0	NULL	question	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To bundle or not to bundle : lawmakers explore the question .
	manualset3
186041	1	415343	7	NULL	NULL	0	NULL	pineal response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To characterize the pineal response to pyridoxine , plasma melatonin was measured in one hundred and twenty children 3 hours after vitamin B6 administration .
	manualset3
186042	2	415343	7	NULL	NULL	0	NULL	 pyridoxine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To characterize the pineal response to pyridoxine , plasma melatonin was measured in one hundred and twenty children 3 hours after vitamin B6 administration .
	manualset3
186044	3	415343	7	NULL	NULL	0	NULL	plasma melatonin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To characterize the pineal response to pyridoxine , plasma melatonin was measured in one hundred and twenty children 3 hours after vitamin B6 administration .
	manualset3
186046	4	415343	7	NULL	NULL	0	NULL	one hundred and twenty children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To characterize the pineal response to pyridoxine , plasma melatonin was measured in one hundred and twenty children 3 hours after vitamin B6 administration .
	manualset3
186047	5	415343	7	NULL	NULL	0	NULL	3 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	To characterize the pineal response to pyridoxine , plasma melatonin was measured in one hundred and twenty children 3 hours after vitamin B6 administration .
	manualset3
186049	6	415343	7	NULL	NULL	NULL	NULL	vitamin B6	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To characterize the pineal response to pyridoxine , plasma melatonin was measured in one hundred and twenty children 3 hours after vitamin B6 administration .
	manualset3
186051	7	415343	7	NULL	NULL	0	NULL	administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To characterize the pineal response to pyridoxine , plasma melatonin was measured in one hundred and twenty children 3 hours after vitamin B6 administration .
	manualset3
186052	1	415344	7	NULL	NULL	0	NULL	reactivity pattern 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To characterize the reactivity pattern of Abs directed to beta2-glycoprotein I ( anti-beta2GPI ) in patients with anti-phospholipid syndrome , we have purified anti-beta2GPI Abs by affinity chromatography using the IgG fractions from sera of five different anti-phospholipid syndrome patients .
	manualset3
186053	2	415344	7	NULL	NULL	0	NULL	Abs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To characterize the reactivity pattern of Abs directed to beta2-glycoprotein I ( anti-beta2GPI ) in patients with anti-phospholipid syndrome , we have purified anti-beta2GPI Abs by affinity chromatography using the IgG fractions from sera of five different anti-phospholipid syndrome patients .
	manualset3
186054	3	415344	7	NULL	NULL	0	NULL	beta2-glycoprotein I ( anti-beta2GPI )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To characterize the reactivity pattern of Abs directed to beta2-glycoprotein I ( anti-beta2GPI ) in patients with anti-phospholipid syndrome , we have purified anti-beta2GPI Abs by affinity chromatography using the IgG fractions from sera of five different anti-phospholipid syndrome patients .
	manualset3
186055	4	415344	7	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To characterize the reactivity pattern of Abs directed to beta2-glycoprotein I ( anti-beta2GPI ) in patients with anti-phospholipid syndrome , we have purified anti-beta2GPI Abs by affinity chromatography using the IgG fractions from sera of five different anti-phospholipid syndrome patients .
	manualset3
186056	5	415344	7	NULL	NULL	0	NULL	anti-phospholipid syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To characterize the reactivity pattern of Abs directed to beta2-glycoprotein I ( anti-beta2GPI ) in patients with anti-phospholipid syndrome , we have purified anti-beta2GPI Abs by affinity chromatography using the IgG fractions from sera of five different anti-phospholipid syndrome patients .
	manualset3
186065	6	415344	7	NULL	NULL	0	NULL	anti-beta2GPI Abs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To characterize the reactivity pattern of Abs directed to beta2-glycoprotein I ( anti-beta2GPI ) in patients with anti-phospholipid syndrome , we have purified anti-beta2GPI Abs by affinity chromatography using the IgG fractions from sera of five different anti-phospholipid syndrome patients .
	manualset3
186067	7	415344	7	NULL	NULL	0	NULL	affinity chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To characterize the reactivity pattern of Abs directed to beta2-glycoprotein I ( anti-beta2GPI ) in patients with anti-phospholipid syndrome , we have purified anti-beta2GPI Abs by affinity chromatography using the IgG fractions from sera of five different anti-phospholipid syndrome patients .
	manualset3
186069	8	415344	7	NULL	NULL	0	NULL	IgG fractions	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	To characterize the reactivity pattern of Abs directed to beta2-glycoprotein I ( anti-beta2GPI ) in patients with anti-phospholipid syndrome , we have purified anti-beta2GPI Abs by affinity chromatography using the IgG fractions from sera of five different anti-phospholipid syndrome patients .
	manualset3
186070	9	415344	7	NULL	NULL	0	NULL	sera 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To characterize the reactivity pattern of Abs directed to beta2-glycoprotein I ( anti-beta2GPI ) in patients with anti-phospholipid syndrome , we have purified anti-beta2GPI Abs by affinity chromatography using the IgG fractions from sera of five different anti-phospholipid syndrome patients .
	manualset3
186072	10	415344	7	NULL	NULL	0	NULL	five	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To characterize the reactivity pattern of Abs directed to beta2-glycoprotein I ( anti-beta2GPI ) in patients with anti-phospholipid syndrome , we have purified anti-beta2GPI Abs by affinity chromatography using the IgG fractions from sera of five different anti-phospholipid syndrome patients .
	manualset3
186073	11	415344	7	NULL	NULL	0	NULL	anti-phospholipid syndrome patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To characterize the reactivity pattern of Abs directed to beta2-glycoprotein I ( anti-beta2GPI ) in patients with anti-phospholipid syndrome , we have purified anti-beta2GPI Abs by affinity chromatography using the IgG fractions from sera of five different anti-phospholipid syndrome patients .
	manualset3
186077	1	415345	7	NULL	NULL	0	NULL	inability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To circumvent the inability of T-DAP12 cells to proliferate following NKG2D ligation by Rae-1beta expressing tumors , DAP12 was engineered into OT-1 cells with an endogenous T cell receptor specific for chicken ovalbumin peptide ( amino acids 257-264 ) .
	manualset3
186079	2	415345	7	NULL	NULL	0	NULL	T-DAP12 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To circumvent the inability of T-DAP12 cells to proliferate following NKG2D ligation by Rae-1beta expressing tumors , DAP12 was engineered into OT-1 cells with an endogenous T cell receptor specific for chicken ovalbumin peptide ( amino acids 257-264 ) .
	manualset3
186080	3	415345	7	NULL	NULL	0	NULL	NKG2D ligation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To circumvent the inability of T-DAP12 cells to proliferate following NKG2D ligation by Rae-1beta expressing tumors , DAP12 was engineered into OT-1 cells with an endogenous T cell receptor specific for chicken ovalbumin peptide ( amino acids 257-264 ) .
	manualset3
186081	4	415345	7	NULL	NULL	0	NULL	Rae-1beta expressing tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To circumvent the inability of T-DAP12 cells to proliferate following NKG2D ligation by Rae-1beta expressing tumors , DAP12 was engineered into OT-1 cells with an endogenous T cell receptor specific for chicken ovalbumin peptide ( amino acids 257-264 ) .
	manualset3
186082	5	415345	7	NULL	NULL	0	NULL	DAP12	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To circumvent the inability of T-DAP12 cells to proliferate following NKG2D ligation by Rae-1beta expressing tumors , DAP12 was engineered into OT-1 cells with an endogenous T cell receptor specific for chicken ovalbumin peptide ( amino acids 257-264 ) .
	manualset3
186083	6	415345	7	NULL	NULL	0	NULL	OT-1 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To circumvent the inability of T-DAP12 cells to proliferate following NKG2D ligation by Rae-1beta expressing tumors , DAP12 was engineered into OT-1 cells with an endogenous T cell receptor specific for chicken ovalbumin peptide ( amino acids 257-264 ) .
	manualset3
186084	7	415345	7	NULL	NULL	0	NULL	endogenous T cell receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To circumvent the inability of T-DAP12 cells to proliferate following NKG2D ligation by Rae-1beta expressing tumors , DAP12 was engineered into OT-1 cells with an endogenous T cell receptor specific for chicken ovalbumin peptide ( amino acids 257-264 ) .
	manualset3
186085	8	415345	7	NULL	NULL	0	NULL	chicken ovalbumin peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	To circumvent the inability of T-DAP12 cells to proliferate following NKG2D ligation by Rae-1beta expressing tumors , DAP12 was engineered into OT-1 cells with an endogenous T cell receptor specific for chicken ovalbumin peptide ( amino acids 257-264 ) .
	manualset3
186087	9	415345	7	NULL	NULL	0	NULL	amino acids 257-264	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To circumvent the inability of T-DAP12 cells to proliferate following NKG2D ligation by Rae-1beta expressing tumors , DAP12 was engineered into OT-1 cells with an endogenous T cell receptor specific for chicken ovalbumin peptide ( amino acids 257-264 ) .
	manualset3
186089	1	415346	7	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify its role , a yeast two-hybrid system ( ths ) screening was utilized to identify Nef cellular partners .
	manualset3
186091	2	415346	7	NULL	NULL	0	NULL	yeast two-hybrid system ( ths ) screening	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify its role , a yeast two-hybrid system ( ths ) screening was utilized to identify Nef cellular partners .
	manualset3
186093	3	415346	7	NULL	NULL	0	NULL	Nef cellular partners 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify its role , a yeast two-hybrid system ( ths ) screening was utilized to identify Nef cellular partners .
	manualset3
186096	1	415347	7	NULL	NULL	0	NULL	Ig structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the Ig structure required for incorporation into ovarian follicles , Ig uptakes were determined after the intravenous injection of chicken and human Igs .
	manualset3
186097	2	415347	7	NULL	NULL	0	NULL	incorporation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the Ig structure required for incorporation into ovarian follicles , Ig uptakes were determined after the intravenous injection of chicken and human Igs .
	manualset3
186098	3	415347	7	NULL	NULL	0	NULL	ovarian follicles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the Ig structure required for incorporation into ovarian follicles , Ig uptakes were determined after the intravenous injection of chicken and human Igs .
	manualset3
186099	4	415347	7	NULL	NULL	0	NULL	Ig uptakes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the Ig structure required for incorporation into ovarian follicles , Ig uptakes were determined after the intravenous injection of chicken and human Igs .
	manualset3
186100	5	415347	7	NULL	NULL	0	NULL	intravenous injection 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the Ig structure required for incorporation into ovarian follicles , Ig uptakes were determined after the intravenous injection of chicken and human Igs .
	manualset3
186101	6	415347	7	NULL	NULL	NULL	NULL	chicken Igs	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To clarify the Ig structure required for incorporation into ovarian follicles , Ig uptakes were determined after the intravenous injection of chicken and human Igs .
	manualset3
186102	7	415347	7	NULL	NULL	NULL	NULL	human Igs	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To clarify the Ig structure required for incorporation into ovarian follicles , Ig uptakes were determined after the intravenous injection of chicken and human Igs .
	manualset3
186105	1	415348	7	NULL	NULL	0	NULL	constitutional changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the importance of the constitutional changes of goblet cell mucins in mucosal defense , euthymic rats were primed by implantation of damaged worms to induce goblet cell changes , and then 3 or 5 days later they were challenged by implantation with normal worms .
	manualset3
186107	2	415348	7	NULL	NULL	NULL	NULL	goblet cell mucins	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To clarify the importance of the constitutional changes of goblet cell mucins in mucosal defense , euthymic rats were primed by implantation of damaged worms to induce goblet cell changes , and then 3 or 5 days later they were challenged by implantation with normal worms .
	manualset3
186113	3	415348	7	NULL	NULL	0	NULL	mucosal defense	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the importance of the constitutional changes of goblet cell mucins in mucosal defense , euthymic rats were primed by implantation of damaged worms to induce goblet cell changes , and then 3 or 5 days later they were challenged by implantation with normal worms .
	manualset3
186114	4	415348	7	NULL	NULL	0	NULL	euthymic rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the importance of the constitutional changes of goblet cell mucins in mucosal defense , euthymic rats were primed by implantation of damaged worms to induce goblet cell changes , and then 3 or 5 days later they were challenged by implantation with normal worms .
	manualset3
186115	5	415348	7	NULL	NULL	0	NULL	implantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the importance of the constitutional changes of goblet cell mucins in mucosal defense , euthymic rats were primed by implantation of damaged worms to induce goblet cell changes , and then 3 or 5 days later they were challenged by implantation with normal worms .
	manualset3
186116	6	415348	7	NULL	NULL	0	NULL	damaged worms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the importance of the constitutional changes of goblet cell mucins in mucosal defense , euthymic rats were primed by implantation of damaged worms to induce goblet cell changes , and then 3 or 5 days later they were challenged by implantation with normal worms .
	manualset3
186117	7	415348	7	NULL	NULL	0	NULL	goblet cell changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the importance of the constitutional changes of goblet cell mucins in mucosal defense , euthymic rats were primed by implantation of damaged worms to induce goblet cell changes , and then 3 or 5 days later they were challenged by implantation with normal worms .
	manualset3
186118	8	415348	7	NULL	NULL	0	NULL	3 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the importance of the constitutional changes of goblet cell mucins in mucosal defense , euthymic rats were primed by implantation of damaged worms to induce goblet cell changes , and then 3 or 5 days later they were challenged by implantation with normal worms .
	manualset3
186120	9	415348	7	NULL	NULL	0	NULL	5 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the importance of the constitutional changes of goblet cell mucins in mucosal defense , euthymic rats were primed by implantation of damaged worms to induce goblet cell changes , and then 3 or 5 days later they were challenged by implantation with normal worms .
	manualset3
186122	10	415348	7	NULL	NULL	0	NULL	implantation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the importance of the constitutional changes of goblet cell mucins in mucosal defense , euthymic rats were primed by implantation of damaged worms to induce goblet cell changes , and then 3 or 5 days later they were challenged by implantation with normal worms .
	manualset3
186123	11	415348	7	NULL	NULL	0	NULL	normal worms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the importance of the constitutional changes of goblet cell mucins in mucosal defense , euthymic rats were primed by implantation of damaged worms to induce goblet cell changes , and then 3 or 5 days later they were challenged by implantation with normal worms .
	manualset3
186133	1	415349	7	NULL	NULL	0	NULL	molecular mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the molecular mechanism underlying the transepidermal extrusion of dermal collagen in acquired perforating dermatosis ( APD ) associated with diabetes mellitus and renal failure , we studied the interaction between advanced glycation end product ( AGE ) - modified extracellular matrix proteins and keratinocytes ( KCs ) in a cell culture system .
	manualset3
186134	2	415349	7	NULL	NULL	0	NULL	transepidermal extrusion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the molecular mechanism underlying the transepidermal extrusion of dermal collagen in acquired perforating dermatosis ( APD ) associated with diabetes mellitus and renal failure , we studied the interaction between advanced glycation end product ( AGE ) - modified extracellular matrix proteins and keratinocytes ( KCs ) in a cell culture system .
	manualset3
186135	3	415349	7	NULL	NULL	0	NULL	dermal collagen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the molecular mechanism underlying the transepidermal extrusion of dermal collagen in acquired perforating dermatosis ( APD ) associated with diabetes mellitus and renal failure , we studied the interaction between advanced glycation end product ( AGE ) - modified extracellular matrix proteins and keratinocytes ( KCs ) in a cell culture system .
	manualset3
186136	4	415349	7	NULL	NULL	0	NULL	acquired perforating dermatosis ( APD ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the molecular mechanism underlying the transepidermal extrusion of dermal collagen in acquired perforating dermatosis ( APD ) associated with diabetes mellitus and renal failure , we studied the interaction between advanced glycation end product ( AGE ) - modified extracellular matrix proteins and keratinocytes ( KCs ) in a cell culture system .
	manualset3
186137	5	415349	7	NULL	NULL	0	NULL	diabetes mellitus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the molecular mechanism underlying the transepidermal extrusion of dermal collagen in acquired perforating dermatosis ( APD ) associated with diabetes mellitus and renal failure , we studied the interaction between advanced glycation end product ( AGE ) - modified extracellular matrix proteins and keratinocytes ( KCs ) in a cell culture system .
	manualset3
186138	6	415349	7	NULL	NULL	0	NULL	renal failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the molecular mechanism underlying the transepidermal extrusion of dermal collagen in acquired perforating dermatosis ( APD ) associated with diabetes mellitus and renal failure , we studied the interaction between advanced glycation end product ( AGE ) - modified extracellular matrix proteins and keratinocytes ( KCs ) in a cell culture system .
	manualset3
186139	7	415349	7	NULL	NULL	0	NULL	 interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the molecular mechanism underlying the transepidermal extrusion of dermal collagen in acquired perforating dermatosis ( APD ) associated with diabetes mellitus and renal failure , we studied the interaction between advanced glycation end product ( AGE ) - modified extracellular matrix proteins and keratinocytes ( KCs ) in a cell culture system .
	manualset3
186140	8	415349	7	NULL	NULL	0	NULL	advanced glycation end product ( AGE ) - modified extracellular matrix proteins 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the molecular mechanism underlying the transepidermal extrusion of dermal collagen in acquired perforating dermatosis ( APD ) associated with diabetes mellitus and renal failure , we studied the interaction between advanced glycation end product ( AGE ) - modified extracellular matrix proteins and keratinocytes ( KCs ) in a cell culture system .
	manualset3
186141	9	415349	7	NULL	NULL	0	NULL	keratinocytes ( KCs )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the molecular mechanism underlying the transepidermal extrusion of dermal collagen in acquired perforating dermatosis ( APD ) associated with diabetes mellitus and renal failure , we studied the interaction between advanced glycation end product ( AGE ) - modified extracellular matrix proteins and keratinocytes ( KCs ) in a cell culture system .
	manualset3
186142	10	415349	7	NULL	NULL	0	NULL	cell culture system	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the molecular mechanism underlying the transepidermal extrusion of dermal collagen in acquired perforating dermatosis ( APD ) associated with diabetes mellitus and renal failure , we studied the interaction between advanced glycation end product ( AGE ) - modified extracellular matrix proteins and keratinocytes ( KCs ) in a cell culture system .
	manualset3
186143	1	415350	7	NULL	NULL	0	NULL	 role 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the role of O2 stores in the fluctuations in VO2 observed with changing posture , O2 intake ( Veo2 ) and pulmonary capillary O2 transfer ( Vpco2 ) were calculated breath by breath with a box-balloon sprometer and mass spectrometer .
	manualset3
186144	2	415350	7	NULL	NULL	0	NULL	O2 stores	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the role of O2 stores in the fluctuations in VO2 observed with changing posture , O2 intake ( Veo2 ) and pulmonary capillary O2 transfer ( Vpco2 ) were calculated breath by breath with a box-balloon sprometer and mass spectrometer .
	manualset3
186145	3	415350	7	NULL	NULL	NULL	NULL	fluctuations in VO2	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To clarify the role of O2 stores in the fluctuations in VO2 observed with changing posture , O2 intake ( Veo2 ) and pulmonary capillary O2 transfer ( Vpco2 ) were calculated breath by breath with a box-balloon sprometer and mass spectrometer .
	manualset3
186147	5	415350	7	NULL	NULL	0	NULL	changing posture	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the role of O2 stores in the fluctuations in VO2 observed with changing posture , O2 intake ( Veo2 ) and pulmonary capillary O2 transfer ( Vpco2 ) were calculated breath by breath with a box-balloon sprometer and mass spectrometer .
	manualset3
186148	6	415350	7	NULL	NULL	0	NULL	O2 intake ( Veo2 )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the role of O2 stores in the fluctuations in VO2 observed with changing posture , O2 intake ( Veo2 ) and pulmonary capillary O2 transfer ( Vpco2 ) were calculated breath by breath with a box-balloon sprometer and mass spectrometer .
	manualset3
186149	7	415350	7	NULL	NULL	0	NULL	pulmonary capillary O2 transfer ( Vpco2 )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the role of O2 stores in the fluctuations in VO2 observed with changing posture , O2 intake ( Veo2 ) and pulmonary capillary O2 transfer ( Vpco2 ) were calculated breath by breath with a box-balloon sprometer and mass spectrometer .
	manualset3
186150	8	415350	7	NULL	NULL	0	NULL	box-balloon sprometer	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the role of O2 stores in the fluctuations in VO2 observed with changing posture , O2 intake ( Veo2 ) and pulmonary capillary O2 transfer ( Vpco2 ) were calculated breath by breath with a box-balloon sprometer and mass spectrometer .
	manualset3
186151	9	415350	7	NULL	NULL	0	NULL	mass spectrometer	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	To clarify the role of O2 stores in the fluctuations in VO2 observed with changing posture , O2 intake ( Veo2 ) and pulmonary capillary O2 transfer ( Vpco2 ) were calculated breath by breath with a box-balloon sprometer and mass spectrometer .
	manualset3
186152	1	415351	7	NULL	NULL	0	NULL	adjustment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After additional adjustment for body mass index and history of diabetes mellitus and hypercholesterolemia , these associations were attenuated and remained statistically significant only for trans FAs ( relative risk in the highest quintile : 1.08 ; 95 % CI : 1.01 to 1.15 ) .
	manualset3
186153	2	415351	7	NULL	NULL	0	NULL	body mass index	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After additional adjustment for body mass index and history of diabetes mellitus and hypercholesterolemia , these associations were attenuated and remained statistically significant only for trans FAs ( relative risk in the highest quintile : 1.08 ; 95 % CI : 1.01 to 1.15 ) .
	manualset3
186154	3	415351	7	NULL	NULL	0	NULL	history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After additional adjustment for body mass index and history of diabetes mellitus and hypercholesterolemia , these associations were attenuated and remained statistically significant only for trans FAs ( relative risk in the highest quintile : 1.08 ; 95 % CI : 1.01 to 1.15 ) .
	manualset3
186155	4	415351	7	NULL	NULL	0	NULL	diabetes mellitus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	After additional adjustment for body mass index and history of diabetes mellitus and hypercholesterolemia , these associations were attenuated and remained statistically significant only for trans FAs ( relative risk in the highest quintile : 1.08 ; 95 % CI : 1.01 to 1.15 ) .
	manualset3
186156	5	415351	7	NULL	NULL	0	NULL	hypercholesterolemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	After additional adjustment for body mass index and history of diabetes mellitus and hypercholesterolemia , these associations were attenuated and remained statistically significant only for trans FAs ( relative risk in the highest quintile : 1.08 ; 95 % CI : 1.01 to 1.15 ) .
	manualset3
186157	6	415351	7	NULL	NULL	0	NULL	associations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	After additional adjustment for body mass index and history of diabetes mellitus and hypercholesterolemia , these associations were attenuated and remained statistically significant only for trans FAs ( relative risk in the highest quintile : 1.08 ; 95 % CI : 1.01 to 1.15 ) .
	manualset3
186158	7	415351	7	NULL	NULL	0	NULL	trans FAs	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After additional adjustment for body mass index and history of diabetes mellitus and hypercholesterolemia , these associations were attenuated and remained statistically significant only for trans FAs ( relative risk in the highest quintile : 1.08 ; 95 % CI : 1.01 to 1.15 ) .
	manualset3
186159	8	415351	7	NULL	NULL	0	NULL	relative risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After additional adjustment for body mass index and history of diabetes mellitus and hypercholesterolemia , these associations were attenuated and remained statistically significant only for trans FAs ( relative risk in the highest quintile : 1.08 ; 95 % CI : 1.01 to 1.15 ) .
	manualset3
186160	9	415351	7	NULL	NULL	0	NULL	highest quintile	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After additional adjustment for body mass index and history of diabetes mellitus and hypercholesterolemia , these associations were attenuated and remained statistically significant only for trans FAs ( relative risk in the highest quintile : 1.08 ; 95 % CI : 1.01 to 1.15 ) .
	manualset3
186161	10	415351	7	NULL	NULL	0	NULL	 1.08	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	After additional adjustment for body mass index and history of diabetes mellitus and hypercholesterolemia , these associations were attenuated and remained statistically significant only for trans FAs ( relative risk in the highest quintile : 1.08 ; 95 % CI : 1.01 to 1.15 ) .
	manualset3
186162	11	415351	7	NULL	NULL	0	NULL	95 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After additional adjustment for body mass index and history of diabetes mellitus and hypercholesterolemia , these associations were attenuated and remained statistically significant only for trans FAs ( relative risk in the highest quintile : 1.08 ; 95 % CI : 1.01 to 1.15 ) .
	manualset3
186163	12	415351	7	NULL	NULL	0	NULL	CI	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After additional adjustment for body mass index and history of diabetes mellitus and hypercholesterolemia , these associations were attenuated and remained statistically significant only for trans FAs ( relative risk in the highest quintile : 1.08 ; 95 % CI : 1.01 to 1.15 ) .
	manualset3
186164	13	415351	7	NULL	NULL	0	NULL	1.01 to 1.15	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	After additional adjustment for body mass index and history of diabetes mellitus and hypercholesterolemia , these associations were attenuated and remained statistically significant only for trans FAs ( relative risk in the highest quintile : 1.08 ; 95 % CI : 1.01 to 1.15 ) .
	manualset3
186165	1	415352	7	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	To collect the data directly from microscope slides , a computer-controlled microscope was integrated with image-processing software to eliminate the need for manual counting and scoring of autoradiograms .
	manualset3
186166	2	415352	7	NULL	NULL	0	NULL	microscope slides	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To collect the data directly from microscope slides , a computer-controlled microscope was integrated with image-processing software to eliminate the need for manual counting and scoring of autoradiograms .
	manualset3
186167	3	415352	7	NULL	NULL	0	NULL	computer-controlled microscope	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	To collect the data directly from microscope slides , a computer-controlled microscope was integrated with image-processing software to eliminate the need for manual counting and scoring of autoradiograms .
	manualset3
186168	4	415352	7	NULL	NULL	0	NULL	 image-processing software	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	To collect the data directly from microscope slides , a computer-controlled microscope was integrated with image-processing software to eliminate the need for manual counting and scoring of autoradiograms .
	manualset3
186169	5	415352	7	NULL	NULL	0	NULL	 manual counting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To collect the data directly from microscope slides , a computer-controlled microscope was integrated with image-processing software to eliminate the need for manual counting and scoring of autoradiograms .
	manualset3
186170	6	415352	7	NULL	NULL	0	NULL	scoring	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To collect the data directly from microscope slides , a computer-controlled microscope was integrated with image-processing software to eliminate the need for manual counting and scoring of autoradiograms .
	manualset3
186171	7	415352	7	NULL	NULL	0	NULL	autoradiograms	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	To collect the data directly from microscope slides , a computer-controlled microscope was integrated with image-processing software to eliminate the need for manual counting and scoring of autoradiograms .
	manualset3
186172	1	415353	7	NULL	NULL	0	NULL	breath and skin exhalation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To compare breath and skin exhalation , minute exhalation volumes per body surface of CO ( VCO ) , NO ( VNO ) and nitrogen oxide ( NO ( x ) , VNO ( x ) ) in breath and skin gas were calculated using gas chromatography with a semiconductor sensor , chemiluminescence method and respiro-monitor .
	manualset3
186173	2	415353	7	NULL	NULL	0	NULL	minute exhalation volumes per body surface	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To compare breath and skin exhalation , minute exhalation volumes per body surface of CO ( VCO ) , NO ( VNO ) and nitrogen oxide ( NO ( x ) , VNO ( x ) ) in breath and skin gas were calculated using gas chromatography with a semiconductor sensor , chemiluminescence method and respiro-monitor .
	manualset3
186174	3	415353	7	NULL	NULL	0	NULL	CO ( VCO )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To compare breath and skin exhalation , minute exhalation volumes per body surface of CO ( VCO ) , NO ( VNO ) and nitrogen oxide ( NO ( x ) , VNO ( x ) ) in breath and skin gas were calculated using gas chromatography with a semiconductor sensor , chemiluminescence method and respiro-monitor .
	manualset3
186175	4	415353	7	NULL	NULL	0	NULL	NO ( VNO )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To compare breath and skin exhalation , minute exhalation volumes per body surface of CO ( VCO ) , NO ( VNO ) and nitrogen oxide ( NO ( x ) , VNO ( x ) ) in breath and skin gas were calculated using gas chromatography with a semiconductor sensor , chemiluminescence method and respiro-monitor .
	manualset3
186176	5	415353	7	NULL	NULL	0	NULL	nitrogen oxide ( NO ( x )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To compare breath and skin exhalation , minute exhalation volumes per body surface of CO ( VCO ) , NO ( VNO ) and nitrogen oxide ( NO ( x ) , VNO ( x ) ) in breath and skin gas were calculated using gas chromatography with a semiconductor sensor , chemiluminescence method and respiro-monitor .
	manualset3
186177	6	415353	7	NULL	NULL	0	NULL	VNO ( x )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To compare breath and skin exhalation , minute exhalation volumes per body surface of CO ( VCO ) , NO ( VNO ) and nitrogen oxide ( NO ( x ) , VNO ( x ) ) in breath and skin gas were calculated using gas chromatography with a semiconductor sensor , chemiluminescence method and respiro-monitor .
	manualset3
186178	7	415353	7	NULL	NULL	0	NULL	breath and skin gas	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To compare breath and skin exhalation , minute exhalation volumes per body surface of CO ( VCO ) , NO ( VNO ) and nitrogen oxide ( NO ( x ) , VNO ( x ) ) in breath and skin gas were calculated using gas chromatography with a semiconductor sensor , chemiluminescence method and respiro-monitor .
	manualset3
186179	8	415353	7	NULL	NULL	0	NULL	gas chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To compare breath and skin exhalation , minute exhalation volumes per body surface of CO ( VCO ) , NO ( VNO ) and nitrogen oxide ( NO ( x ) , VNO ( x ) ) in breath and skin gas were calculated using gas chromatography with a semiconductor sensor , chemiluminescence method and respiro-monitor .
	manualset3
186180	9	415353	7	NULL	NULL	0	NULL	semiconductor sensor	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	To compare breath and skin exhalation , minute exhalation volumes per body surface of CO ( VCO ) , NO ( VNO ) and nitrogen oxide ( NO ( x ) , VNO ( x ) ) in breath and skin gas were calculated using gas chromatography with a semiconductor sensor , chemiluminescence method and respiro-monitor .
	manualset3
186181	10	415353	7	NULL	NULL	0	NULL	chemiluminescence method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To compare breath and skin exhalation , minute exhalation volumes per body surface of CO ( VCO ) , NO ( VNO ) and nitrogen oxide ( NO ( x ) , VNO ( x ) ) in breath and skin gas were calculated using gas chromatography with a semiconductor sensor , chemiluminescence method and respiro-monitor .
	manualset3
186182	11	415353	7	NULL	NULL	0	NULL	respiro-monitor	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	To compare breath and skin exhalation , minute exhalation volumes per body surface of CO ( VCO ) , NO ( VNO ) and nitrogen oxide ( NO ( x ) , VNO ( x ) ) in breath and skin gas were calculated using gas chromatography with a semiconductor sensor , chemiluminescence method and respiro-monitor .
	manualset3
186183	1	415354	7	NULL	NULL	0	NULL	methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To compare methods of calculating facility service levels for outpatient wound centers and to demonstrate the advantages of an acuity-based billing system ( one that incorporates components of facility work that is non-reimbursable by procedure codes and that represents an activity-based costing approach to medical billing ) , a retrospective study of 5 , 098 patient encounters contained in a wound care-specific electronic medical record database was conducted .
	manualset3
186184	2	415354	7	NULL	NULL	0	NULL	facility service levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To compare methods of calculating facility service levels for outpatient wound centers and to demonstrate the advantages of an acuity-based billing system ( one that incorporates components of facility work that is non-reimbursable by procedure codes and that represents an activity-based costing approach to medical billing ) , a retrospective study of 5 , 098 patient encounters contained in a wound care-specific electronic medical record database was conducted .
	manualset3
186185	3	415354	7	NULL	NULL	0	NULL	outpatient wound centers	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	To compare methods of calculating facility service levels for outpatient wound centers and to demonstrate the advantages of an acuity-based billing system ( one that incorporates components of facility work that is non-reimbursable by procedure codes and that represents an activity-based costing approach to medical billing ) , a retrospective study of 5 , 098 patient encounters contained in a wound care-specific electronic medical record database was conducted .
	manualset3
186186	4	415354	7	NULL	NULL	0	NULL	advantages	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To compare methods of calculating facility service levels for outpatient wound centers and to demonstrate the advantages of an acuity-based billing system ( one that incorporates components of facility work that is non-reimbursable by procedure codes and that represents an activity-based costing approach to medical billing ) , a retrospective study of 5 , 098 patient encounters contained in a wound care-specific electronic medical record database was conducted .
	manualset3
186187	5	415354	7	NULL	NULL	0	NULL	acuity-based billing system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	To compare methods of calculating facility service levels for outpatient wound centers and to demonstrate the advantages of an acuity-based billing system ( one that incorporates components of facility work that is non-reimbursable by procedure codes and that represents an activity-based costing approach to medical billing ) , a retrospective study of 5 , 098 patient encounters contained in a wound care-specific electronic medical record database was conducted .
	manualset3
186188	6	415354	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To compare methods of calculating facility service levels for outpatient wound centers and to demonstrate the advantages of an acuity-based billing system ( one that incorporates components of facility work that is non-reimbursable by procedure codes and that represents an activity-based costing approach to medical billing ) , a retrospective study of 5 , 098 patient encounters contained in a wound care-specific electronic medical record database was conducted .
	manualset3
186189	7	415354	7	NULL	NULL	0	NULL	components	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To compare methods of calculating facility service levels for outpatient wound centers and to demonstrate the advantages of an acuity-based billing system ( one that incorporates components of facility work that is non-reimbursable by procedure codes and that represents an activity-based costing approach to medical billing ) , a retrospective study of 5 , 098 patient encounters contained in a wound care-specific electronic medical record database was conducted .
	manualset3
186190	8	415354	7	NULL	NULL	0	NULL	facility work	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	To compare methods of calculating facility service levels for outpatient wound centers and to demonstrate the advantages of an acuity-based billing system ( one that incorporates components of facility work that is non-reimbursable by procedure codes and that represents an activity-based costing approach to medical billing ) , a retrospective study of 5 , 098 patient encounters contained in a wound care-specific electronic medical record database was conducted .
	manualset3
186191	9	415354	7	NULL	NULL	0	NULL	 non-reimbursable	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To compare methods of calculating facility service levels for outpatient wound centers and to demonstrate the advantages of an acuity-based billing system ( one that incorporates components of facility work that is non-reimbursable by procedure codes and that represents an activity-based costing approach to medical billing ) , a retrospective study of 5 , 098 patient encounters contained in a wound care-specific electronic medical record database was conducted .
	manualset3
186192	10	415354	7	NULL	NULL	0	NULL	procedure codes 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	To compare methods of calculating facility service levels for outpatient wound centers and to demonstrate the advantages of an acuity-based billing system ( one that incorporates components of facility work that is non-reimbursable by procedure codes and that represents an activity-based costing approach to medical billing ) , a retrospective study of 5 , 098 patient encounters contained in a wound care-specific electronic medical record database was conducted .
	manualset3
186193	11	415354	7	NULL	NULL	0	NULL	activity-based costing approach 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To compare methods of calculating facility service levels for outpatient wound centers and to demonstrate the advantages of an acuity-based billing system ( one that incorporates components of facility work that is non-reimbursable by procedure codes and that represents an activity-based costing approach to medical billing ) , a retrospective study of 5 , 098 patient encounters contained in a wound care-specific electronic medical record database was conducted .
	manualset3
186194	12	415354	7	NULL	NULL	0	NULL	 medical billing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To compare methods of calculating facility service levels for outpatient wound centers and to demonstrate the advantages of an acuity-based billing system ( one that incorporates components of facility work that is non-reimbursable by procedure codes and that represents an activity-based costing approach to medical billing ) , a retrospective study of 5 , 098 patient encounters contained in a wound care-specific electronic medical record database was conducted .
	manualset3
186195	13	415354	7	NULL	NULL	0	NULL	retrospective study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To compare methods of calculating facility service levels for outpatient wound centers and to demonstrate the advantages of an acuity-based billing system ( one that incorporates components of facility work that is non-reimbursable by procedure codes and that represents an activity-based costing approach to medical billing ) , a retrospective study of 5 , 098 patient encounters contained in a wound care-specific electronic medical record database was conducted .
	manualset3
186196	14	415354	7	NULL	NULL	0	NULL	5 , 098 patient encounters	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To compare methods of calculating facility service levels for outpatient wound centers and to demonstrate the advantages of an acuity-based billing system ( one that incorporates components of facility work that is non-reimbursable by procedure codes and that represents an activity-based costing approach to medical billing ) , a retrospective study of 5 , 098 patient encounters contained in a wound care-specific electronic medical record database was conducted .
	manualset3
186197	15	415354	7	NULL	NULL	0	NULL	wound care-specific electronic medical record database	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	To compare methods of calculating facility service levels for outpatient wound centers and to demonstrate the advantages of an acuity-based billing system ( one that incorporates components of facility work that is non-reimbursable by procedure codes and that represents an activity-based costing approach to medical billing ) , a retrospective study of 5 , 098 patient encounters contained in a wound care-specific electronic medical record database was conducted .
	manualset3
186198	1	415355	7	NULL	NULL	0	NULL	hospital administrators	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To compete effectively , hospital administrators need to define their businesses and markets and assess their position within those markets .
	manualset3
186199	2	415355	7	NULL	NULL	0	NULL	businesses	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To compete effectively , hospital administrators need to define their businesses and markets and assess their position within those markets .
	manualset3
186200	3	415355	7	NULL	NULL	0	NULL	markets	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To compete effectively , hospital administrators need to define their businesses and markets and assess their position within those markets .
	manualset3
186201	4	415355	7	NULL	NULL	0	NULL	position 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To compete effectively , hospital administrators need to define their businesses and markets and assess their position within those markets .
	manualset3
186202	5	415355	7	NULL	NULL	0	NULL	markets	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To compete effectively , hospital administrators need to define their businesses and markets and assess their position within those markets .
	manualset3
186203	1	415356	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To confirm the findings in intact cells , we studied Cas , a Src substrate that possesses SH2 and SH3 ligands .
	manualset3
186204	2	415356	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To confirm the findings in intact cells , we studied Cas , a Src substrate that possesses SH2 and SH3 ligands .
	manualset3
186205	3	415356	7	NULL	NULL	0	NULL	Cas	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To confirm the findings in intact cells , we studied Cas , a Src substrate that possesses SH2 and SH3 ligands .
	manualset3
186206	4	415356	7	NULL	NULL	0	NULL	Src substrate	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To confirm the findings in intact cells , we studied Cas , a Src substrate that possesses SH2 and SH3 ligands .
	manualset3
186207	5	415356	7	NULL	NULL	0	NULL	SH2 ligands	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To confirm the findings in intact cells , we studied Cas , a Src substrate that possesses SH2 and SH3 ligands .
	manualset3
186208	6	415356	7	NULL	NULL	0	NULL	SH3 ligands	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To confirm the findings in intact cells , we studied Cas , a Src substrate that possesses SH2 and SH3 ligands .
	manualset3
186209	1	415357	7	NULL	NULL	0	NULL	learned lessons	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To convey learned lessons from the Hiroshima experience , three books are helpful : `` A-bomb Mayor '' by Shinzo Hamai , `` The Meaning of Survival '' compiled by the Chugoku Shimbun and `` The Children of the A-bomb '' compiled by Arata Osada .
	manualset3
186210	2	415357	7	NULL	NULL	0	NULL	Hiroshima experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To convey learned lessons from the Hiroshima experience , three books are helpful : `` A-bomb Mayor '' by Shinzo Hamai , `` The Meaning of Survival '' compiled by the Chugoku Shimbun and `` The Children of the A-bomb '' compiled by Arata Osada .
	manualset3
186211	3	415357	7	NULL	NULL	0	NULL	three books	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	To convey learned lessons from the Hiroshima experience , three books are helpful : `` A-bomb Mayor '' by Shinzo Hamai , `` The Meaning of Survival '' compiled by the Chugoku Shimbun and `` The Children of the A-bomb '' compiled by Arata Osada .
	manualset3
186212	4	415357	7	NULL	NULL	0	NULL	 `` A-bomb Mayor ''	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	To convey learned lessons from the Hiroshima experience , three books are helpful : `` A-bomb Mayor '' by Shinzo Hamai , `` The Meaning of Survival '' compiled by the Chugoku Shimbun and `` The Children of the A-bomb '' compiled by Arata Osada .
	manualset3
186213	5	415357	7	NULL	NULL	0	NULL	 Shinzo Hamai	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	To convey learned lessons from the Hiroshima experience , three books are helpful : `` A-bomb Mayor '' by Shinzo Hamai , `` The Meaning of Survival '' compiled by the Chugoku Shimbun and `` The Children of the A-bomb '' compiled by Arata Osada .
	manualset3
186214	6	415357	7	NULL	NULL	0	NULL	`` The Meaning of Survival ''	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	To convey learned lessons from the Hiroshima experience , three books are helpful : `` A-bomb Mayor '' by Shinzo Hamai , `` The Meaning of Survival '' compiled by the Chugoku Shimbun and `` The Children of the A-bomb '' compiled by Arata Osada .
	manualset3
186215	7	415357	7	NULL	NULL	0	NULL	Chugoku Shimbun 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	To convey learned lessons from the Hiroshima experience , three books are helpful : `` A-bomb Mayor '' by Shinzo Hamai , `` The Meaning of Survival '' compiled by the Chugoku Shimbun and `` The Children of the A-bomb '' compiled by Arata Osada .
	manualset3
186216	8	415357	7	NULL	NULL	0	NULL	`` The Children of the A-bomb ''	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	To convey learned lessons from the Hiroshima experience , three books are helpful : `` A-bomb Mayor '' by Shinzo Hamai , `` The Meaning of Survival '' compiled by the Chugoku Shimbun and `` The Children of the A-bomb '' compiled by Arata Osada .
	manualset3
186217	9	415357	7	NULL	NULL	0	NULL	Arata Osada 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	To convey learned lessons from the Hiroshima experience , three books are helpful : `` A-bomb Mayor '' by Shinzo Hamai , `` The Meaning of Survival '' compiled by the Chugoku Shimbun and `` The Children of the A-bomb '' compiled by Arata Osada .
	manualset3
186218	1	415358	7	NULL	NULL	NULL	NULL	codes	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To cope with the impact of codes , design , and attitudes in a renovation project , a hospital may have to make compromises and consider many alternatives to its plan .
	manualset3
186219	2	415358	7	NULL	NULL	0	NULL	design	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To cope with the impact of codes , design , and attitudes in a renovation project , a hospital may have to make compromises and consider many alternatives to its plan .
	manualset3
186220	3	415358	7	NULL	NULL	NULL	NULL	renovation project	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To cope with the impact of codes , design , and attitudes in a renovation project , a hospital may have to make compromises and consider many alternatives to its plan .
	manualset3
186221	4	415358	7	NULL	NULL	0	NULL	hospital	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	To cope with the impact of codes , design , and attitudes in a renovation project , a hospital may have to make compromises and consider many alternatives to its plan .
	manualset3
186222	5	415358	7	NULL	NULL	0	NULL	plan	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To cope with the impact of codes , design , and attitudes in a renovation project , a hospital may have to make compromises and consider many alternatives to its plan .
	manualset3
186223	6	415358	7	NULL	NULL	0	NULL	impact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To cope with the impact of codes , design , and attitudes in a renovation project , a hospital may have to make compromises and consider many alternatives to its plan .
	manualset3
186224	7	415358	7	NULL	NULL	0	NULL	attitudes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To cope with the impact of codes , design , and attitudes in a renovation project , a hospital may have to make compromises and consider many alternatives to its plan .
	manualset3
186225	1	415359	7	NULL	NULL	0	NULL	covariates	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjusting for covariates , DDE and PCB were both positively associated with BMI and inversely with BMI-gain ; they were lowest with low BMI , high BMI-gain , and longer lactation .
	manualset3
186226	2	415359	7	NULL	NULL	0	NULL	DDE	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjusting for covariates , DDE and PCB were both positively associated with BMI and inversely with BMI-gain ; they were lowest with low BMI , high BMI-gain , and longer lactation .
	manualset3
186227	3	415359	7	NULL	NULL	0	NULL	PCB	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjusting for covariates , DDE and PCB were both positively associated with BMI and inversely with BMI-gain ; they were lowest with low BMI , high BMI-gain , and longer lactation .
	manualset3
186228	4	415359	7	NULL	NULL	0	NULL	BMI 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjusting for covariates , DDE and PCB were both positively associated with BMI and inversely with BMI-gain ; they were lowest with low BMI , high BMI-gain , and longer lactation .
	manualset3
186229	5	415359	7	NULL	NULL	0	NULL	BMI-gain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjusting for covariates , DDE and PCB were both positively associated with BMI and inversely with BMI-gain ; they were lowest with low BMI , high BMI-gain , and longer lactation .
	manualset3
186230	6	415359	7	NULL	NULL	0	NULL	 low BMI	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjusting for covariates , DDE and PCB were both positively associated with BMI and inversely with BMI-gain ; they were lowest with low BMI , high BMI-gain , and longer lactation .
	manualset3
186231	7	415359	7	NULL	NULL	0	NULL	high BMI-gain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjusting for covariates , DDE and PCB were both positively associated with BMI and inversely with BMI-gain ; they were lowest with low BMI , high BMI-gain , and longer lactation .
	manualset3
186232	8	415359	7	NULL	NULL	0	NULL	longer lactation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjusting for covariates , DDE and PCB were both positively associated with BMI and inversely with BMI-gain ; they were lowest with low BMI , high BMI-gain , and longer lactation .
	manualset3
186233	1	415360	7	NULL	NULL	NULL	NULL	 date	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To date , only patients with ischemic heart disease ( IHD ) have been investigated .
	manualset3
186234	2	415360	7	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To date , only patients with ischemic heart disease ( IHD ) have been investigated .
	manualset3
186235	3	415360	7	NULL	NULL	0	NULL	 ischemic heart disease ( IHD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To date , only patients with ischemic heart disease ( IHD ) have been investigated .
	manualset3
186385	1	415361	7	NULL	NULL	0	NULL	 date	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	To date , several enzymatic reactions , including Polymerase Chain Reaction , Rolling Circle - and Strand Displacement Amplification for signal enhancement of nucleic acid biosensors , have been presented .
	manualset3
186387	2	415361	7	NULL	NULL	0	NULL	enzymatic reactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To date , several enzymatic reactions , including Polymerase Chain Reaction , Rolling Circle - and Strand Displacement Amplification for signal enhancement of nucleic acid biosensors , have been presented .
	manualset3
186390	3	415361	7	NULL	NULL	0	NULL	Polymerase Chain Reaction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To date , several enzymatic reactions , including Polymerase Chain Reaction , Rolling Circle - and Strand Displacement Amplification for signal enhancement of nucleic acid biosensors , have been presented .
	manualset3
186392	4	415361	7	NULL	NULL	0	NULL	Rolling Circle - and Strand Displacement Amplification 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To date , several enzymatic reactions , including Polymerase Chain Reaction , Rolling Circle - and Strand Displacement Amplification for signal enhancement of nucleic acid biosensors , have been presented .
	manualset3
186396	5	415361	7	NULL	NULL	0	NULL	signal enhancement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To date , several enzymatic reactions , including Polymerase Chain Reaction , Rolling Circle - and Strand Displacement Amplification for signal enhancement of nucleic acid biosensors , have been presented .
	manualset3
186399	6	415361	7	NULL	NULL	0	NULL	nucleic acid biosensors	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	To date , several enzymatic reactions , including Polymerase Chain Reaction , Rolling Circle - and Strand Displacement Amplification for signal enhancement of nucleic acid biosensors , have been presented .
	manualset3
186403	1	415362	7	NULL	NULL	0	NULL	date	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	To date , the function of MADS-domain transcription factors in non-seed plants remains largely elusive , although a number of genes have been isolated and characterized from a variety of species .
	manualset3
186404	2	415362	7	NULL	NULL	0	NULL	function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To date , the function of MADS-domain transcription factors in non-seed plants remains largely elusive , although a number of genes have been isolated and characterized from a variety of species .
	manualset3
186406	3	415362	7	NULL	NULL	0	NULL	MADS-domain transcription factors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To date , the function of MADS-domain transcription factors in non-seed plants remains largely elusive , although a number of genes have been isolated and characterized from a variety of species .
	manualset3
186407	4	415362	7	NULL	NULL	0	NULL	non-seed plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To date , the function of MADS-domain transcription factors in non-seed plants remains largely elusive , although a number of genes have been isolated and characterized from a variety of species .
	manualset3
186408	5	415362	7	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To date , the function of MADS-domain transcription factors in non-seed plants remains largely elusive , although a number of genes have been isolated and characterized from a variety of species .
	manualset3
186409	6	415362	7	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To date , the function of MADS-domain transcription factors in non-seed plants remains largely elusive , although a number of genes have been isolated and characterized from a variety of species .
	manualset3
186410	7	415362	7	NULL	NULL	0	NULL	variety	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To date , the function of MADS-domain transcription factors in non-seed plants remains largely elusive , although a number of genes have been isolated and characterized from a variety of species .
	manualset3
186411	8	415362	7	NULL	NULL	0	NULL	species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To date , the function of MADS-domain transcription factors in non-seed plants remains largely elusive , although a number of genes have been isolated and characterized from a variety of species .
	manualset3
186425	1	415363	7	NULL	NULL	0	NULL	date	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	To date , the origin of the band and its effect on polyethylene chemical and mechanical properties , and hence , clinical performance , have not been confirmed , and correlations between radiation sterilization and clinical wear have not been made .
	manualset3
186426	2	415363	7	NULL	NULL	NULL	NULL	 origin of the band	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To date , the origin of the band and its effect on polyethylene chemical and mechanical properties , and hence , clinical performance , have not been confirmed , and correlations between radiation sterilization and clinical wear have not been made .
	manualset3
186427	3	415363	7	NULL	NULL	NULL	NULL	effect	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To date , the origin of the band and its effect on polyethylene chemical and mechanical properties , and hence , clinical performance , have not been confirmed , and correlations between radiation sterilization and clinical wear have not been made .
	manualset3
186428	4	415363	7	NULL	NULL	NULL	NULL	polyethylene chemical properties	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To date , the origin of the band and its effect on polyethylene chemical and mechanical properties , and hence , clinical performance , have not been confirmed , and correlations between radiation sterilization and clinical wear have not been made .
	manualset3
186429	5	415363	7	NULL	NULL	0	NULL	mechanical properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To date , the origin of the band and its effect on polyethylene chemical and mechanical properties , and hence , clinical performance , have not been confirmed , and correlations between radiation sterilization and clinical wear have not been made .
	manualset3
186430	6	415363	7	NULL	NULL	0	NULL	clinical performance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To date , the origin of the band and its effect on polyethylene chemical and mechanical properties , and hence , clinical performance , have not been confirmed , and correlations between radiation sterilization and clinical wear have not been made .
	manualset3
186431	7	415363	7	NULL	NULL	0	NULL	correlations 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	To date , the origin of the band and its effect on polyethylene chemical and mechanical properties , and hence , clinical performance , have not been confirmed , and correlations between radiation sterilization and clinical wear have not been made .
	manualset3
186432	8	415363	7	NULL	NULL	0	NULL	radiation sterilization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To date , the origin of the band and its effect on polyethylene chemical and mechanical properties , and hence , clinical performance , have not been confirmed , and correlations between radiation sterilization and clinical wear have not been made .
	manualset3
186433	9	415363	7	NULL	NULL	0	NULL	clinical wear	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To date , the origin of the band and its effect on polyethylene chemical and mechanical properties , and hence , clinical performance , have not been confirmed , and correlations between radiation sterilization and clinical wear have not been made .
	manualset3
186434	1	415364	7	NULL	NULL	0	NULL	 date	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	To date , there has been no chronological age estimation according to third-molar mineralization in eastern Turkish children and adolescents .
	manualset3
186435	2	415364	7	NULL	NULL	0	NULL	chronological age estimation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To date , there has been no chronological age estimation according to third-molar mineralization in eastern Turkish children and adolescents .
	manualset3
186436	3	415364	7	NULL	NULL	0	NULL	third-molar mineralization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To date , there has been no chronological age estimation according to third-molar mineralization in eastern Turkish children and adolescents .
	manualset3
186437	4	415364	7	NULL	NULL	0	NULL	eastern Turkish children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To date , there has been no chronological age estimation according to third-molar mineralization in eastern Turkish children and adolescents .
	manualset3
186438	5	415364	7	NULL	NULL	0	NULL	 adolescents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To date , there has been no chronological age estimation according to third-molar mineralization in eastern Turkish children and adolescents .
	manualset3
186439	1	415365	7	NULL	NULL	0	NULL	potential confounders	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjusting for potential confounders , both BNP and apelin retained their statistical significance as independent predictors of arrhythmia recurrence .
	manualset3
186440	2	415365	7	NULL	NULL	0	NULL	BNP	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjusting for potential confounders , both BNP and apelin retained their statistical significance as independent predictors of arrhythmia recurrence .
	manualset3
186441	3	415365	7	NULL	NULL	0	NULL	apelin	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjusting for potential confounders , both BNP and apelin retained their statistical significance as independent predictors of arrhythmia recurrence .
	manualset3
186442	4	415365	7	NULL	NULL	0	NULL	statistical significance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjusting for potential confounders , both BNP and apelin retained their statistical significance as independent predictors of arrhythmia recurrence .
	manualset3
186443	5	415365	7	NULL	NULL	0	NULL	 independent predictors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjusting for potential confounders , both BNP and apelin retained their statistical significance as independent predictors of arrhythmia recurrence .
	manualset3
186444	6	415365	7	NULL	NULL	0	NULL	arrhythmia recurrence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjusting for potential confounders , both BNP and apelin retained their statistical significance as independent predictors of arrhythmia recurrence .
	manualset3
186445	1	415366	7	NULL	NULL	0	NULL	 entry mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To define the entry mechanism of HIV-1 complexed with anti-HIV-1 antibody , we attempted to determine the receptor molecules responsible for mediating enhancement of HIV-1 infection of monocytic cells .
	manualset3
186446	2	415366	7	NULL	NULL	0	NULL	HIV-1	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To define the entry mechanism of HIV-1 complexed with anti-HIV-1 antibody , we attempted to determine the receptor molecules responsible for mediating enhancement of HIV-1 infection of monocytic cells .
	manualset3
186447	3	415366	7	NULL	NULL	0	NULL	anti-HIV-1 antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To define the entry mechanism of HIV-1 complexed with anti-HIV-1 antibody , we attempted to determine the receptor molecules responsible for mediating enhancement of HIV-1 infection of monocytic cells .
	manualset3
186448	4	415366	7	NULL	NULL	0	NULL	receptor molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	To define the entry mechanism of HIV-1 complexed with anti-HIV-1 antibody , we attempted to determine the receptor molecules responsible for mediating enhancement of HIV-1 infection of monocytic cells .
	manualset3
186449	5	415366	7	NULL	NULL	0	NULL	enhancement	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To define the entry mechanism of HIV-1 complexed with anti-HIV-1 antibody , we attempted to determine the receptor molecules responsible for mediating enhancement of HIV-1 infection of monocytic cells .
	manualset3
186450	6	415366	7	NULL	NULL	0	NULL	HIV-1 infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To define the entry mechanism of HIV-1 complexed with anti-HIV-1 antibody , we attempted to determine the receptor molecules responsible for mediating enhancement of HIV-1 infection of monocytic cells .
	manualset3
186451	7	415366	7	NULL	NULL	0	NULL	monocytic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To define the entry mechanism of HIV-1 complexed with anti-HIV-1 antibody , we attempted to determine the receptor molecules responsible for mediating enhancement of HIV-1 infection of monocytic cells .
	manualset3
186452	1	415367	7	NULL	NULL	0	NULL	 role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To define the role of p0071 in junction assembly , p0071 was tested for interactions with other components of the endothelial junctional complex .
	manualset3
186453	2	415367	7	NULL	NULL	0	NULL	 p0071	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To define the role of p0071 in junction assembly , p0071 was tested for interactions with other components of the endothelial junctional complex .
	manualset3
186454	3	415367	7	NULL	NULL	0	NULL	 junction assembly	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To define the role of p0071 in junction assembly , p0071 was tested for interactions with other components of the endothelial junctional complex .
	manualset3
186455	4	415367	7	NULL	NULL	0	NULL	p0071	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To define the role of p0071 in junction assembly , p0071 was tested for interactions with other components of the endothelial junctional complex .
	manualset3
186456	5	415367	7	NULL	NULL	0	NULL	interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To define the role of p0071 in junction assembly , p0071 was tested for interactions with other components of the endothelial junctional complex .
	manualset3
186457	6	415367	7	NULL	NULL	0	NULL	components	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To define the role of p0071 in junction assembly , p0071 was tested for interactions with other components of the endothelial junctional complex .
	manualset3
186458	7	415367	7	NULL	NULL	0	NULL	endothelial junctional complex	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To define the role of p0071 in junction assembly , p0071 was tested for interactions with other components of the endothelial junctional complex .
	manualset3
186472	1	415368	7	NULL	NULL	0	NULL	mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To delineate the underlying mechanism , we conducted a yeast two-hybrid screening and identified IRSp53S , a protein critical in cell mobilization , as one of the Eps8-binding partners from a human brain cDNA library .
	manualset3
186473	2	415368	7	NULL	NULL	0	NULL	yeast two-hybrid screening	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To delineate the underlying mechanism , we conducted a yeast two-hybrid screening and identified IRSp53S , a protein critical in cell mobilization , as one of the Eps8-binding partners from a human brain cDNA library .
	manualset3
186474	3	415368	7	NULL	NULL	0	NULL	IRSp53S	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To delineate the underlying mechanism , we conducted a yeast two-hybrid screening and identified IRSp53S , a protein critical in cell mobilization , as one of the Eps8-binding partners from a human brain cDNA library .
	manualset3
186475	4	415368	7	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To delineate the underlying mechanism , we conducted a yeast two-hybrid screening and identified IRSp53S , a protein critical in cell mobilization , as one of the Eps8-binding partners from a human brain cDNA library .
	manualset3
186476	5	415368	7	NULL	NULL	0	NULL	cell mobilization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To delineate the underlying mechanism , we conducted a yeast two-hybrid screening and identified IRSp53S , a protein critical in cell mobilization , as one of the Eps8-binding partners from a human brain cDNA library .
	manualset3
186477	6	415368	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To delineate the underlying mechanism , we conducted a yeast two-hybrid screening and identified IRSp53S , a protein critical in cell mobilization , as one of the Eps8-binding partners from a human brain cDNA library .
	manualset3
186478	7	415368	7	NULL	NULL	0	NULL	Eps8-binding partner	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To delineate the underlying mechanism , we conducted a yeast two-hybrid screening and identified IRSp53S , a protein critical in cell mobilization , as one of the Eps8-binding partners from a human brain cDNA library .
	manualset3
186479	8	415368	7	NULL	NULL	0	NULL	human brain cDNA library 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To delineate the underlying mechanism , we conducted a yeast two-hybrid screening and identified IRSp53S , a protein critical in cell mobilization , as one of the Eps8-binding partners from a human brain cDNA library .
	manualset3
186605	1	415369	7	NULL	NULL	0	NULL	utility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To demonstrate the utility of these ultrathin , fracture-free substrates , lipid bilayer membranes composed of phosphorylated derivatives of phosphoinositides ( PIs ) were deposited on the new substrates for biosensing applications .
	manualset3
186606	2	415369	7	NULL	NULL	0	NULL	ultrathin , fracture-free substrates	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To demonstrate the utility of these ultrathin , fracture-free substrates , lipid bilayer membranes composed of phosphorylated derivatives of phosphoinositides ( PIs ) were deposited on the new substrates for biosensing applications .
	manualset3
186607	3	415369	7	NULL	NULL	0	NULL	lipid bilayer membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	To demonstrate the utility of these ultrathin , fracture-free substrates , lipid bilayer membranes composed of phosphorylated derivatives of phosphoinositides ( PIs ) were deposited on the new substrates for biosensing applications .
	manualset3
186608	4	415369	7	NULL	NULL	0	NULL	phosphorylated derivatives	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To demonstrate the utility of these ultrathin , fracture-free substrates , lipid bilayer membranes composed of phosphorylated derivatives of phosphoinositides ( PIs ) were deposited on the new substrates for biosensing applications .
	manualset3
186609	5	415369	7	NULL	NULL	0	NULL	phosphoinositides ( PIs )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To demonstrate the utility of these ultrathin , fracture-free substrates , lipid bilayer membranes composed of phosphorylated derivatives of phosphoinositides ( PIs ) were deposited on the new substrates for biosensing applications .
	manualset3
186610	6	415369	7	NULL	NULL	0	NULL	new substrates	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To demonstrate the utility of these ultrathin , fracture-free substrates , lipid bilayer membranes composed of phosphorylated derivatives of phosphoinositides ( PIs ) were deposited on the new substrates for biosensing applications .
	manualset3
186611	7	415369	7	NULL	NULL	0	NULL	biosensing applications	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To demonstrate the utility of these ultrathin , fracture-free substrates , lipid bilayer membranes composed of phosphorylated derivatives of phosphoinositides ( PIs ) were deposited on the new substrates for biosensing applications .
	manualset3
186612	1	415370	7	NULL	NULL	0	NULL	antibody-binding sequences	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To detect antibody-binding sequences on Ara h1 , we synthesized a series of peptides of the Ara h1 protein on a multi-pin apparatus for the pin-peptide ELISA .
	manualset3
186613	2	415370	7	NULL	NULL	0	NULL	Ara h1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To detect antibody-binding sequences on Ara h1 , we synthesized a series of peptides of the Ara h1 protein on a multi-pin apparatus for the pin-peptide ELISA .
	manualset3
186614	3	415370	7	NULL	NULL	0	NULL	series of peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	To detect antibody-binding sequences on Ara h1 , we synthesized a series of peptides of the Ara h1 protein on a multi-pin apparatus for the pin-peptide ELISA .
	manualset3
186615	4	415370	7	NULL	NULL	0	NULL	Ara h1 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To detect antibody-binding sequences on Ara h1 , we synthesized a series of peptides of the Ara h1 protein on a multi-pin apparatus for the pin-peptide ELISA .
	manualset3
186616	5	415370	7	NULL	NULL	0	NULL	 multi-pin apparatus 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	To detect antibody-binding sequences on Ara h1 , we synthesized a series of peptides of the Ara h1 protein on a multi-pin apparatus for the pin-peptide ELISA .
	manualset3
186617	6	415370	7	NULL	NULL	0	NULL	pin-peptide ELISA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To detect antibody-binding sequences on Ara h1 , we synthesized a series of peptides of the Ara h1 protein on a multi-pin apparatus for the pin-peptide ELISA .
	manualset3
186618	1	415371	7	NULL	NULL	0	NULL	promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine if this promoter is sufficient to direct expression to the suprabasal cells of stratified squamous epithelia in vivo , we have now generated transgenic mouse lines harboring the involucrin promoter sequences linked to a beta-galactosidase reporter gene .
	manualset3
186619	2	415371	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine if this promoter is sufficient to direct expression to the suprabasal cells of stratified squamous epithelia in vivo , we have now generated transgenic mouse lines harboring the involucrin promoter sequences linked to a beta-galactosidase reporter gene .
	manualset3
186620	3	415371	7	NULL	NULL	0	NULL	suprabasal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine if this promoter is sufficient to direct expression to the suprabasal cells of stratified squamous epithelia in vivo , we have now generated transgenic mouse lines harboring the involucrin promoter sequences linked to a beta-galactosidase reporter gene .
	manualset3
186621	4	415371	7	NULL	NULL	0	NULL	stratified squamous epithelia	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine if this promoter is sufficient to direct expression to the suprabasal cells of stratified squamous epithelia in vivo , we have now generated transgenic mouse lines harboring the involucrin promoter sequences linked to a beta-galactosidase reporter gene .
	manualset3
186622	5	415371	7	NULL	NULL	0	NULL	transgenic mouse lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine if this promoter is sufficient to direct expression to the suprabasal cells of stratified squamous epithelia in vivo , we have now generated transgenic mouse lines harboring the involucrin promoter sequences linked to a beta-galactosidase reporter gene .
	manualset3
186623	6	415371	7	NULL	NULL	0	NULL	involucrin promoter sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine if this promoter is sufficient to direct expression to the suprabasal cells of stratified squamous epithelia in vivo , we have now generated transgenic mouse lines harboring the involucrin promoter sequences linked to a beta-galactosidase reporter gene .
	manualset3
186624	7	415371	7	NULL	NULL	0	NULL	beta-galactosidase reporter gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine if this promoter is sufficient to direct expression to the suprabasal cells of stratified squamous epithelia in vivo , we have now generated transgenic mouse lines harboring the involucrin promoter sequences linked to a beta-galactosidase reporter gene .
	manualset3
186625	1	415372	7	NULL	NULL	0	NULL	cellular mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the cellular mechanism or mechanisms by which parathyroid hormone analogs antagonize pressor effects , we examined the effect of these peptides on angiotensin II-induced calcium mobilization in fura 2-AM-loaded cultured rat vascular smooth muscle cells .
	manualset3
186626	2	415372	7	NULL	NULL	0	NULL	mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the cellular mechanism or mechanisms by which parathyroid hormone analogs antagonize pressor effects , we examined the effect of these peptides on angiotensin II-induced calcium mobilization in fura 2-AM-loaded cultured rat vascular smooth muscle cells .
	manualset3
186627	3	415372	7	NULL	NULL	0	NULL	parathyroid hormone analogs	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the cellular mechanism or mechanisms by which parathyroid hormone analogs antagonize pressor effects , we examined the effect of these peptides on angiotensin II-induced calcium mobilization in fura 2-AM-loaded cultured rat vascular smooth muscle cells .
	manualset3
186628	4	415372	7	NULL	NULL	0	NULL	pressor effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the cellular mechanism or mechanisms by which parathyroid hormone analogs antagonize pressor effects , we examined the effect of these peptides on angiotensin II-induced calcium mobilization in fura 2-AM-loaded cultured rat vascular smooth muscle cells .
	manualset3
186629	5	415372	7	NULL	NULL	0	NULL	effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the cellular mechanism or mechanisms by which parathyroid hormone analogs antagonize pressor effects , we examined the effect of these peptides on angiotensin II-induced calcium mobilization in fura 2-AM-loaded cultured rat vascular smooth muscle cells .
	manualset3
186630	6	415372	7	NULL	NULL	0	NULL	peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the cellular mechanism or mechanisms by which parathyroid hormone analogs antagonize pressor effects , we examined the effect of these peptides on angiotensin II-induced calcium mobilization in fura 2-AM-loaded cultured rat vascular smooth muscle cells .
	manualset3
186631	7	415372	7	NULL	NULL	0	NULL	angiotensin II-induced calcium mobilization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the cellular mechanism or mechanisms by which parathyroid hormone analogs antagonize pressor effects , we examined the effect of these peptides on angiotensin II-induced calcium mobilization in fura 2-AM-loaded cultured rat vascular smooth muscle cells .
	manualset3
186632	8	415372	7	NULL	NULL	0	NULL	fura 2-AM-loaded cultured rat vascular smooth muscle cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the cellular mechanism or mechanisms by which parathyroid hormone analogs antagonize pressor effects , we examined the effect of these peptides on angiotensin II-induced calcium mobilization in fura 2-AM-loaded cultured rat vascular smooth muscle cells .
	manualset3
186633	1	415373	7	NULL	NULL	0	NULL	 degree	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the degree of intraspecimen fecal egg count variation in Schistosoma mansoni infection and its impact on commonly used parasitologic parameters obtained by single egg counts , 10 25-mg Kato-Katz slides were prepared from each of three stool specimens collected on different days in a study group of 20 infected people .
	manualset3
186634	2	415373	7	NULL	NULL	NULL	NULL	intraspecimen fecal egg count variation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To determine the degree of intraspecimen fecal egg count variation in Schistosoma mansoni infection and its impact on commonly used parasitologic parameters obtained by single egg counts , 10 25-mg Kato-Katz slides were prepared from each of three stool specimens collected on different days in a study group of 20 infected people .
	manualset3
186635	3	415373	7	NULL	NULL	0	NULL	Schistosoma mansoni infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the degree of intraspecimen fecal egg count variation in Schistosoma mansoni infection and its impact on commonly used parasitologic parameters obtained by single egg counts , 10 25-mg Kato-Katz slides were prepared from each of three stool specimens collected on different days in a study group of 20 infected people .
	manualset3
186636	4	415373	7	NULL	NULL	0	NULL	 impact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the degree of intraspecimen fecal egg count variation in Schistosoma mansoni infection and its impact on commonly used parasitologic parameters obtained by single egg counts , 10 25-mg Kato-Katz slides were prepared from each of three stool specimens collected on different days in a study group of 20 infected people .
	manualset3
186637	5	415373	7	NULL	NULL	0	NULL	parasitologic parameters	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the degree of intraspecimen fecal egg count variation in Schistosoma mansoni infection and its impact on commonly used parasitologic parameters obtained by single egg counts , 10 25-mg Kato-Katz slides were prepared from each of three stool specimens collected on different days in a study group of 20 infected people .
	manualset3
186638	6	415373	7	NULL	NULL	0	NULL	single egg counts 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the degree of intraspecimen fecal egg count variation in Schistosoma mansoni infection and its impact on commonly used parasitologic parameters obtained by single egg counts , 10 25-mg Kato-Katz slides were prepared from each of three stool specimens collected on different days in a study group of 20 infected people .
	manualset3
186639	7	415373	7	NULL	NULL	0	NULL	10 25-mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the degree of intraspecimen fecal egg count variation in Schistosoma mansoni infection and its impact on commonly used parasitologic parameters obtained by single egg counts , 10 25-mg Kato-Katz slides were prepared from each of three stool specimens collected on different days in a study group of 20 infected people .
	manualset3
186640	8	415373	7	NULL	NULL	0	NULL	Kato-Katz slides	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the degree of intraspecimen fecal egg count variation in Schistosoma mansoni infection and its impact on commonly used parasitologic parameters obtained by single egg counts , 10 25-mg Kato-Katz slides were prepared from each of three stool specimens collected on different days in a study group of 20 infected people .
	manualset3
186641	9	415373	7	NULL	NULL	0	NULL	 three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the degree of intraspecimen fecal egg count variation in Schistosoma mansoni infection and its impact on commonly used parasitologic parameters obtained by single egg counts , 10 25-mg Kato-Katz slides were prepared from each of three stool specimens collected on different days in a study group of 20 infected people .
	manualset3
186642	10	415373	7	NULL	NULL	0	NULL	stool specimens	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the degree of intraspecimen fecal egg count variation in Schistosoma mansoni infection and its impact on commonly used parasitologic parameters obtained by single egg counts , 10 25-mg Kato-Katz slides were prepared from each of three stool specimens collected on different days in a study group of 20 infected people .
	manualset3
186643	11	415373	7	NULL	NULL	0	NULL	different days	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the degree of intraspecimen fecal egg count variation in Schistosoma mansoni infection and its impact on commonly used parasitologic parameters obtained by single egg counts , 10 25-mg Kato-Katz slides were prepared from each of three stool specimens collected on different days in a study group of 20 infected people .
	manualset3
186644	12	415373	7	NULL	NULL	0	NULL	study group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the degree of intraspecimen fecal egg count variation in Schistosoma mansoni infection and its impact on commonly used parasitologic parameters obtained by single egg counts , 10 25-mg Kato-Katz slides were prepared from each of three stool specimens collected on different days in a study group of 20 infected people .
	manualset3
186645	13	415373	7	NULL	NULL	0	NULL	20	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the degree of intraspecimen fecal egg count variation in Schistosoma mansoni infection and its impact on commonly used parasitologic parameters obtained by single egg counts , 10 25-mg Kato-Katz slides were prepared from each of three stool specimens collected on different days in a study group of 20 infected people .
	manualset3
186646	14	415373	7	NULL	NULL	0	NULL	infected people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the degree of intraspecimen fecal egg count variation in Schistosoma mansoni infection and its impact on commonly used parasitologic parameters obtained by single egg counts , 10 25-mg Kato-Katz slides were prepared from each of three stool specimens collected on different days in a study group of 20 infected people .
	manualset3
186647	1	415374	7	NULL	NULL	0	NULL	smoking status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjusting for smoking status , carrying the putative `` high-risk '' genotype combination , the faster metabolism of PAH-epoxides to PAH-diol-epoxides ( CYP1B1 432Val/Val and mEH 139Arg/Arg ) with lower PAH-diol-epoxide conjugation ( GSTP1 ( 105 ) Ile/Ile ) , was associated with increased adducts only in Caucasian nontumor cells ( 0.2363 + / - 0.0132 versus 0.1920 + / - 0.0157 ; P = 0.05 ) .
	manualset3
186648	2	415374	7	NULL	NULL	0	NULL	putative `` high-risk '' genotype combination	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjusting for smoking status , carrying the putative `` high-risk '' genotype combination , the faster metabolism of PAH-epoxides to PAH-diol-epoxides ( CYP1B1 432Val/Val and mEH 139Arg/Arg ) with lower PAH-diol-epoxide conjugation ( GSTP1 ( 105 ) Ile/Ile ) , was associated with increased adducts only in Caucasian nontumor cells ( 0.2363 + / - 0.0132 versus 0.1920 + / - 0.0157 ; P = 0.05 ) .
	manualset3
186649	3	415374	7	NULL	NULL	NULL	NULL	faster metabolism	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After adjusting for smoking status , carrying the putative `` high-risk '' genotype combination , the faster metabolism of PAH-epoxides to PAH-diol-epoxides ( CYP1B1 432Val/Val and mEH 139Arg/Arg ) with lower PAH-diol-epoxide conjugation ( GSTP1 ( 105 ) Ile/Ile ) , was associated with increased adducts only in Caucasian nontumor cells ( 0.2363 + / - 0.0132 versus 0.1920 + / - 0.0157 ; P = 0.05 ) .
	manualset3
186650	4	415374	7	NULL	NULL	0	NULL	PAH-epoxides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjusting for smoking status , carrying the putative `` high-risk '' genotype combination , the faster metabolism of PAH-epoxides to PAH-diol-epoxides ( CYP1B1 432Val/Val and mEH 139Arg/Arg ) with lower PAH-diol-epoxide conjugation ( GSTP1 ( 105 ) Ile/Ile ) , was associated with increased adducts only in Caucasian nontumor cells ( 0.2363 + / - 0.0132 versus 0.1920 + / - 0.0157 ; P = 0.05 ) .
	manualset3
186651	5	415374	7	NULL	NULL	0	NULL	 PAH-diol-epoxides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjusting for smoking status , carrying the putative `` high-risk '' genotype combination , the faster metabolism of PAH-epoxides to PAH-diol-epoxides ( CYP1B1 432Val/Val and mEH 139Arg/Arg ) with lower PAH-diol-epoxide conjugation ( GSTP1 ( 105 ) Ile/Ile ) , was associated with increased adducts only in Caucasian nontumor cells ( 0.2363 + / - 0.0132 versus 0.1920 + / - 0.0157 ; P = 0.05 ) .
	manualset3
186652	6	415374	7	NULL	NULL	0	NULL	CYP1B1 432Val/Val 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjusting for smoking status , carrying the putative `` high-risk '' genotype combination , the faster metabolism of PAH-epoxides to PAH-diol-epoxides ( CYP1B1 432Val/Val and mEH 139Arg/Arg ) with lower PAH-diol-epoxide conjugation ( GSTP1 ( 105 ) Ile/Ile ) , was associated with increased adducts only in Caucasian nontumor cells ( 0.2363 + / - 0.0132 versus 0.1920 + / - 0.0157 ; P = 0.05 ) .
	manualset3
186653	7	415374	7	NULL	NULL	0	NULL	mEH 139Arg/Arg	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjusting for smoking status , carrying the putative `` high-risk '' genotype combination , the faster metabolism of PAH-epoxides to PAH-diol-epoxides ( CYP1B1 432Val/Val and mEH 139Arg/Arg ) with lower PAH-diol-epoxide conjugation ( GSTP1 ( 105 ) Ile/Ile ) , was associated with increased adducts only in Caucasian nontumor cells ( 0.2363 + / - 0.0132 versus 0.1920 + / - 0.0157 ; P = 0.05 ) .
	manualset3
186654	8	415374	7	NULL	NULL	0	NULL	lower PAH-diol-epoxide conjugation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjusting for smoking status , carrying the putative `` high-risk '' genotype combination , the faster metabolism of PAH-epoxides to PAH-diol-epoxides ( CYP1B1 432Val/Val and mEH 139Arg/Arg ) with lower PAH-diol-epoxide conjugation ( GSTP1 ( 105 ) Ile/Ile ) , was associated with increased adducts only in Caucasian nontumor cells ( 0.2363 + / - 0.0132 versus 0.1920 + / - 0.0157 ; P = 0.05 ) .
	manualset3
186655	9	415374	7	NULL	NULL	0	NULL	GSTP1 ( 105 ) Ile/Ile	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjusting for smoking status , carrying the putative `` high-risk '' genotype combination , the faster metabolism of PAH-epoxides to PAH-diol-epoxides ( CYP1B1 432Val/Val and mEH 139Arg/Arg ) with lower PAH-diol-epoxide conjugation ( GSTP1 ( 105 ) Ile/Ile ) , was associated with increased adducts only in Caucasian nontumor cells ( 0.2363 + / - 0.0132 versus 0.1920 + / - 0.0157 ; P = 0.05 ) .
	manualset3
186656	10	415374	7	NULL	NULL	0	NULL	 increased adducts	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjusting for smoking status , carrying the putative `` high-risk '' genotype combination , the faster metabolism of PAH-epoxides to PAH-diol-epoxides ( CYP1B1 432Val/Val and mEH 139Arg/Arg ) with lower PAH-diol-epoxide conjugation ( GSTP1 ( 105 ) Ile/Ile ) , was associated with increased adducts only in Caucasian nontumor cells ( 0.2363 + / - 0.0132 versus 0.1920 + / - 0.0157 ; P = 0.05 ) .
	manualset3
186657	11	415374	7	NULL	NULL	0	NULL	Caucasian nontumor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjusting for smoking status , carrying the putative `` high-risk '' genotype combination , the faster metabolism of PAH-epoxides to PAH-diol-epoxides ( CYP1B1 432Val/Val and mEH 139Arg/Arg ) with lower PAH-diol-epoxide conjugation ( GSTP1 ( 105 ) Ile/Ile ) , was associated with increased adducts only in Caucasian nontumor cells ( 0.2363 + / - 0.0132 versus 0.1920 + / - 0.0157 ; P = 0.05 ) .
	manualset3
186658	12	415374	7	NULL	NULL	0	NULL	0.2363 + / - 0.0132	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjusting for smoking status , carrying the putative `` high-risk '' genotype combination , the faster metabolism of PAH-epoxides to PAH-diol-epoxides ( CYP1B1 432Val/Val and mEH 139Arg/Arg ) with lower PAH-diol-epoxide conjugation ( GSTP1 ( 105 ) Ile/Ile ) , was associated with increased adducts only in Caucasian nontumor cells ( 0.2363 + / - 0.0132 versus 0.1920 + / - 0.0157 ; P = 0.05 ) .
	manualset3
186659	13	415374	7	NULL	NULL	0	NULL	0.1920 + / - 0.0157	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjusting for smoking status , carrying the putative `` high-risk '' genotype combination , the faster metabolism of PAH-epoxides to PAH-diol-epoxides ( CYP1B1 432Val/Val and mEH 139Arg/Arg ) with lower PAH-diol-epoxide conjugation ( GSTP1 ( 105 ) Ile/Ile ) , was associated with increased adducts only in Caucasian nontumor cells ( 0.2363 + / - 0.0132 versus 0.1920 + / - 0.0157 ; P = 0.05 ) .
	manualset3
186660	14	415374	7	NULL	NULL	0	NULL	P = 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjusting for smoking status , carrying the putative `` high-risk '' genotype combination , the faster metabolism of PAH-epoxides to PAH-diol-epoxides ( CYP1B1 432Val/Val and mEH 139Arg/Arg ) with lower PAH-diol-epoxide conjugation ( GSTP1 ( 105 ) Ile/Ile ) , was associated with increased adducts only in Caucasian nontumor cells ( 0.2363 + / - 0.0132 versus 0.1920 + / - 0.0157 ; P = 0.05 ) .
	manualset3
186661	1	415375	7	NULL	NULL	0	NULL	effect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effect of benzodiazepine premedication on central nervous system and cardiovascular effects of bupivacaine , the authors administered toxic doses of bupivacaine to awake spontaneously breathing pigs after intravenous premedication with midazolam ( 0.06 mg/kg ) , diazepam ( 0.15 mg/kg ) , or saline .
	manualset3
186662	2	415375	7	NULL	NULL	0	NULL	benzodiazepine premedication	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effect of benzodiazepine premedication on central nervous system and cardiovascular effects of bupivacaine , the authors administered toxic doses of bupivacaine to awake spontaneously breathing pigs after intravenous premedication with midazolam ( 0.06 mg/kg ) , diazepam ( 0.15 mg/kg ) , or saline .
	manualset3
186663	3	415375	7	NULL	NULL	0	NULL	central nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effect of benzodiazepine premedication on central nervous system and cardiovascular effects of bupivacaine , the authors administered toxic doses of bupivacaine to awake spontaneously breathing pigs after intravenous premedication with midazolam ( 0.06 mg/kg ) , diazepam ( 0.15 mg/kg ) , or saline .
	manualset3
186664	4	415375	7	NULL	NULL	0	NULL	cardiovascular effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effect of benzodiazepine premedication on central nervous system and cardiovascular effects of bupivacaine , the authors administered toxic doses of bupivacaine to awake spontaneously breathing pigs after intravenous premedication with midazolam ( 0.06 mg/kg ) , diazepam ( 0.15 mg/kg ) , or saline .
	manualset3
186665	5	415375	7	NULL	NULL	0	NULL	bupivacaine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effect of benzodiazepine premedication on central nervous system and cardiovascular effects of bupivacaine , the authors administered toxic doses of bupivacaine to awake spontaneously breathing pigs after intravenous premedication with midazolam ( 0.06 mg/kg ) , diazepam ( 0.15 mg/kg ) , or saline .
	manualset3
186666	6	415375	7	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effect of benzodiazepine premedication on central nervous system and cardiovascular effects of bupivacaine , the authors administered toxic doses of bupivacaine to awake spontaneously breathing pigs after intravenous premedication with midazolam ( 0.06 mg/kg ) , diazepam ( 0.15 mg/kg ) , or saline .
	manualset3
186667	7	415375	7	NULL	NULL	0	NULL	toxic doses	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effect of benzodiazepine premedication on central nervous system and cardiovascular effects of bupivacaine , the authors administered toxic doses of bupivacaine to awake spontaneously breathing pigs after intravenous premedication with midazolam ( 0.06 mg/kg ) , diazepam ( 0.15 mg/kg ) , or saline .
	manualset3
186668	8	415375	7	NULL	NULL	0	NULL	bupivacaine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effect of benzodiazepine premedication on central nervous system and cardiovascular effects of bupivacaine , the authors administered toxic doses of bupivacaine to awake spontaneously breathing pigs after intravenous premedication with midazolam ( 0.06 mg/kg ) , diazepam ( 0.15 mg/kg ) , or saline .
	manualset3
186669	9	415375	7	NULL	NULL	0	NULL	breathing pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effect of benzodiazepine premedication on central nervous system and cardiovascular effects of bupivacaine , the authors administered toxic doses of bupivacaine to awake spontaneously breathing pigs after intravenous premedication with midazolam ( 0.06 mg/kg ) , diazepam ( 0.15 mg/kg ) , or saline .
	manualset3
186670	10	415375	7	NULL	NULL	0	NULL	 intravenous premedication	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effect of benzodiazepine premedication on central nervous system and cardiovascular effects of bupivacaine , the authors administered toxic doses of bupivacaine to awake spontaneously breathing pigs after intravenous premedication with midazolam ( 0.06 mg/kg ) , diazepam ( 0.15 mg/kg ) , or saline .
	manualset3
186671	11	415375	7	NULL	NULL	0	NULL	midazolam	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effect of benzodiazepine premedication on central nervous system and cardiovascular effects of bupivacaine , the authors administered toxic doses of bupivacaine to awake spontaneously breathing pigs after intravenous premedication with midazolam ( 0.06 mg/kg ) , diazepam ( 0.15 mg/kg ) , or saline .
	manualset3
186672	12	415375	7	NULL	NULL	0	NULL	 0.06 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effect of benzodiazepine premedication on central nervous system and cardiovascular effects of bupivacaine , the authors administered toxic doses of bupivacaine to awake spontaneously breathing pigs after intravenous premedication with midazolam ( 0.06 mg/kg ) , diazepam ( 0.15 mg/kg ) , or saline .
	manualset3
186673	13	415375	7	NULL	NULL	0	NULL	diazepam	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effect of benzodiazepine premedication on central nervous system and cardiovascular effects of bupivacaine , the authors administered toxic doses of bupivacaine to awake spontaneously breathing pigs after intravenous premedication with midazolam ( 0.06 mg/kg ) , diazepam ( 0.15 mg/kg ) , or saline .
	manualset3
186674	14	415375	7	NULL	NULL	0	NULL	0.15 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effect of benzodiazepine premedication on central nervous system and cardiovascular effects of bupivacaine , the authors administered toxic doses of bupivacaine to awake spontaneously breathing pigs after intravenous premedication with midazolam ( 0.06 mg/kg ) , diazepam ( 0.15 mg/kg ) , or saline .
	manualset3
186675	15	415375	7	NULL	NULL	0	NULL	saline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effect of benzodiazepine premedication on central nervous system and cardiovascular effects of bupivacaine , the authors administered toxic doses of bupivacaine to awake spontaneously breathing pigs after intravenous premedication with midazolam ( 0.06 mg/kg ) , diazepam ( 0.15 mg/kg ) , or saline .
	manualset3
186676	1	415376	7	NULL	NULL	0	NULL	effect of surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effect of surgery on subsequent clinical course , we reviewed the treatment records of 30 patients with known stage IV carcinoma of the kidney who underwent nephrectomy or additional procedures in preparation for systemic therapy .
	manualset3
186677	2	415376	7	NULL	NULL	0	NULL	clinical course	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effect of surgery on subsequent clinical course , we reviewed the treatment records of 30 patients with known stage IV carcinoma of the kidney who underwent nephrectomy or additional procedures in preparation for systemic therapy .
	manualset3
186678	3	415376	7	NULL	NULL	0	NULL	 treatment records	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effect of surgery on subsequent clinical course , we reviewed the treatment records of 30 patients with known stage IV carcinoma of the kidney who underwent nephrectomy or additional procedures in preparation for systemic therapy .
	manualset3
186679	4	415376	7	NULL	NULL	0	NULL	30 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effect of surgery on subsequent clinical course , we reviewed the treatment records of 30 patients with known stage IV carcinoma of the kidney who underwent nephrectomy or additional procedures in preparation for systemic therapy .
	manualset3
186680	5	415376	7	NULL	NULL	0	NULL	stage IV carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effect of surgery on subsequent clinical course , we reviewed the treatment records of 30 patients with known stage IV carcinoma of the kidney who underwent nephrectomy or additional procedures in preparation for systemic therapy .
	manualset3
186681	6	415376	7	NULL	NULL	0	NULL	kidney	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effect of surgery on subsequent clinical course , we reviewed the treatment records of 30 patients with known stage IV carcinoma of the kidney who underwent nephrectomy or additional procedures in preparation for systemic therapy .
	manualset3
186682	7	415376	7	NULL	NULL	0	NULL	nephrectomy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effect of surgery on subsequent clinical course , we reviewed the treatment records of 30 patients with known stage IV carcinoma of the kidney who underwent nephrectomy or additional procedures in preparation for systemic therapy .
	manualset3
186683	8	415376	7	NULL	NULL	0	NULL	procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effect of surgery on subsequent clinical course , we reviewed the treatment records of 30 patients with known stage IV carcinoma of the kidney who underwent nephrectomy or additional procedures in preparation for systemic therapy .
	manualset3
186684	9	415376	7	NULL	NULL	0	NULL	preparation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effect of surgery on subsequent clinical course , we reviewed the treatment records of 30 patients with known stage IV carcinoma of the kidney who underwent nephrectomy or additional procedures in preparation for systemic therapy .
	manualset3
186685	10	415376	7	NULL	NULL	0	NULL	systemic therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effect of surgery on subsequent clinical course , we reviewed the treatment records of 30 patients with known stage IV carcinoma of the kidney who underwent nephrectomy or additional procedures in preparation for systemic therapy .
	manualset3
186686	1	415377	7	NULL	NULL	0	NULL	 effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effects of Ca2 + antagonism in vivo , we examined the influence of nifedipine on the Aldo response to Na + depletion and K + loading in 11 healthy subjects .
	manualset3
186687	2	415377	7	NULL	NULL	0	NULL	Ca2 + antagonism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effects of Ca2 + antagonism in vivo , we examined the influence of nifedipine on the Aldo response to Na + depletion and K + loading in 11 healthy subjects .
	manualset3
186688	3	415377	7	NULL	NULL	0	NULL	influence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effects of Ca2 + antagonism in vivo , we examined the influence of nifedipine on the Aldo response to Na + depletion and K + loading in 11 healthy subjects .
	manualset3
186689	4	415377	7	NULL	NULL	0	NULL	nifedipine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effects of Ca2 + antagonism in vivo , we examined the influence of nifedipine on the Aldo response to Na + depletion and K + loading in 11 healthy subjects .
	manualset3
186690	5	415377	7	NULL	NULL	0	NULL	Aldo response 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effects of Ca2 + antagonism in vivo , we examined the influence of nifedipine on the Aldo response to Na + depletion and K + loading in 11 healthy subjects .
	manualset3
186691	6	415377	7	NULL	NULL	0	NULL	Na + depletion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effects of Ca2 + antagonism in vivo , we examined the influence of nifedipine on the Aldo response to Na + depletion and K + loading in 11 healthy subjects .
	manualset3
186692	7	415377	7	NULL	NULL	0	NULL	K + loading 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effects of Ca2 + antagonism in vivo , we examined the influence of nifedipine on the Aldo response to Na + depletion and K + loading in 11 healthy subjects .
	manualset3
186693	8	415377	7	NULL	NULL	0	NULL	 11	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effects of Ca2 + antagonism in vivo , we examined the influence of nifedipine on the Aldo response to Na + depletion and K + loading in 11 healthy subjects .
	manualset3
186694	9	415377	7	NULL	NULL	0	NULL	healthy subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the effects of Ca2 + antagonism in vivo , we examined the influence of nifedipine on the Aldo response to Na + depletion and K + loading in 11 healthy subjects .
	manualset3
186695	1	415378	7	NULL	NULL	0	NULL	existence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the existence and histological distribution of cell subpopulations with numerical chromosome aberrations , interphase cytogenetic analysis using probes specific for chromosomes 1 , X , and Y was applied to paraffin tissue sections of 23 cases : 12 cases of complete mole , 3 cases of partial mole , and 8 cases of abortions .
	manualset3
186696	2	415378	7	NULL	NULL	0	NULL	histological distribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the existence and histological distribution of cell subpopulations with numerical chromosome aberrations , interphase cytogenetic analysis using probes specific for chromosomes 1 , X , and Y was applied to paraffin tissue sections of 23 cases : 12 cases of complete mole , 3 cases of partial mole , and 8 cases of abortions .
	manualset3
186697	3	415378	7	NULL	NULL	0	NULL	cell subpopulations	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the existence and histological distribution of cell subpopulations with numerical chromosome aberrations , interphase cytogenetic analysis using probes specific for chromosomes 1 , X , and Y was applied to paraffin tissue sections of 23 cases : 12 cases of complete mole , 3 cases of partial mole , and 8 cases of abortions .
	manualset3
186698	4	415378	7	NULL	NULL	0	NULL	numerical chromosome aberrations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the existence and histological distribution of cell subpopulations with numerical chromosome aberrations , interphase cytogenetic analysis using probes specific for chromosomes 1 , X , and Y was applied to paraffin tissue sections of 23 cases : 12 cases of complete mole , 3 cases of partial mole , and 8 cases of abortions .
	manualset3
186699	5	415378	7	NULL	NULL	0	NULL	interphase cytogenetic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the existence and histological distribution of cell subpopulations with numerical chromosome aberrations , interphase cytogenetic analysis using probes specific for chromosomes 1 , X , and Y was applied to paraffin tissue sections of 23 cases : 12 cases of complete mole , 3 cases of partial mole , and 8 cases of abortions .
	manualset3
186700	6	415378	7	NULL	NULL	0	NULL	probes	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the existence and histological distribution of cell subpopulations with numerical chromosome aberrations , interphase cytogenetic analysis using probes specific for chromosomes 1 , X , and Y was applied to paraffin tissue sections of 23 cases : 12 cases of complete mole , 3 cases of partial mole , and 8 cases of abortions .
	manualset3
186701	7	415378	7	NULL	NULL	0	NULL	chromosomes 1 	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the existence and histological distribution of cell subpopulations with numerical chromosome aberrations , interphase cytogenetic analysis using probes specific for chromosomes 1 , X , and Y was applied to paraffin tissue sections of 23 cases : 12 cases of complete mole , 3 cases of partial mole , and 8 cases of abortions .
	manualset3
186702	8	415378	7	NULL	NULL	0	NULL	chromosomes X	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the existence and histological distribution of cell subpopulations with numerical chromosome aberrations , interphase cytogenetic analysis using probes specific for chromosomes 1 , X , and Y was applied to paraffin tissue sections of 23 cases : 12 cases of complete mole , 3 cases of partial mole , and 8 cases of abortions .
	manualset3
186703	9	415378	7	NULL	NULL	0	NULL	chromosomes Y	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the existence and histological distribution of cell subpopulations with numerical chromosome aberrations , interphase cytogenetic analysis using probes specific for chromosomes 1 , X , and Y was applied to paraffin tissue sections of 23 cases : 12 cases of complete mole , 3 cases of partial mole , and 8 cases of abortions .
	manualset3
186704	10	415378	7	NULL	NULL	0	NULL	paraffin tissue sections	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the existence and histological distribution of cell subpopulations with numerical chromosome aberrations , interphase cytogenetic analysis using probes specific for chromosomes 1 , X , and Y was applied to paraffin tissue sections of 23 cases : 12 cases of complete mole , 3 cases of partial mole , and 8 cases of abortions .
	manualset3
186705	11	415378	7	NULL	NULL	0	NULL	 23 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the existence and histological distribution of cell subpopulations with numerical chromosome aberrations , interphase cytogenetic analysis using probes specific for chromosomes 1 , X , and Y was applied to paraffin tissue sections of 23 cases : 12 cases of complete mole , 3 cases of partial mole , and 8 cases of abortions .
	manualset3
186706	12	415378	7	NULL	NULL	0	NULL	 12 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the existence and histological distribution of cell subpopulations with numerical chromosome aberrations , interphase cytogenetic analysis using probes specific for chromosomes 1 , X , and Y was applied to paraffin tissue sections of 23 cases : 12 cases of complete mole , 3 cases of partial mole , and 8 cases of abortions .
	manualset3
186707	13	415378	7	NULL	NULL	0	NULL	complete mole	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the existence and histological distribution of cell subpopulations with numerical chromosome aberrations , interphase cytogenetic analysis using probes specific for chromosomes 1 , X , and Y was applied to paraffin tissue sections of 23 cases : 12 cases of complete mole , 3 cases of partial mole , and 8 cases of abortions .
	manualset3
186708	14	415378	7	NULL	NULL	0	NULL	3 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the existence and histological distribution of cell subpopulations with numerical chromosome aberrations , interphase cytogenetic analysis using probes specific for chromosomes 1 , X , and Y was applied to paraffin tissue sections of 23 cases : 12 cases of complete mole , 3 cases of partial mole , and 8 cases of abortions .
	manualset3
186709	15	415378	7	NULL	NULL	0	NULL	partial mole	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the existence and histological distribution of cell subpopulations with numerical chromosome aberrations , interphase cytogenetic analysis using probes specific for chromosomes 1 , X , and Y was applied to paraffin tissue sections of 23 cases : 12 cases of complete mole , 3 cases of partial mole , and 8 cases of abortions .
	manualset3
186710	16	415378	7	NULL	NULL	0	NULL	 8 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the existence and histological distribution of cell subpopulations with numerical chromosome aberrations , interphase cytogenetic analysis using probes specific for chromosomes 1 , X , and Y was applied to paraffin tissue sections of 23 cases : 12 cases of complete mole , 3 cases of partial mole , and 8 cases of abortions .
	manualset3
186711	17	415378	7	NULL	NULL	0	NULL	abortions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the existence and histological distribution of cell subpopulations with numerical chromosome aberrations , interphase cytogenetic analysis using probes specific for chromosomes 1 , X , and Y was applied to paraffin tissue sections of 23 cases : 12 cases of complete mole , 3 cases of partial mole , and 8 cases of abortions .
	manualset3
186712	1	415379	7	NULL	NULL	0	NULL	mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the mechanism of action of AGT-2 , we used a bovine granulosa cell model in which luteinizing hormone ( LH ) increased the expression of genes essential for ovulation in a time - and dose-dependent manner .
	manualset3
186713	2	415379	7	NULL	NULL	0	NULL	action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the mechanism of action of AGT-2 , we used a bovine granulosa cell model in which luteinizing hormone ( LH ) increased the expression of genes essential for ovulation in a time - and dose-dependent manner .
	manualset3
186714	3	415379	7	NULL	NULL	0	NULL	AGT-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the mechanism of action of AGT-2 , we used a bovine granulosa cell model in which luteinizing hormone ( LH ) increased the expression of genes essential for ovulation in a time - and dose-dependent manner .
	manualset3
186715	4	415379	7	NULL	NULL	0	NULL	bovine granulosa cell model	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the mechanism of action of AGT-2 , we used a bovine granulosa cell model in which luteinizing hormone ( LH ) increased the expression of genes essential for ovulation in a time - and dose-dependent manner .
	manualset3
186716	5	415379	7	NULL	NULL	0	NULL	luteinizing hormone ( LH )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the mechanism of action of AGT-2 , we used a bovine granulosa cell model in which luteinizing hormone ( LH ) increased the expression of genes essential for ovulation in a time - and dose-dependent manner .
	manualset3
186717	6	415379	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the mechanism of action of AGT-2 , we used a bovine granulosa cell model in which luteinizing hormone ( LH ) increased the expression of genes essential for ovulation in a time - and dose-dependent manner .
	manualset3
186718	7	415379	7	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the mechanism of action of AGT-2 , we used a bovine granulosa cell model in which luteinizing hormone ( LH ) increased the expression of genes essential for ovulation in a time - and dose-dependent manner .
	manualset3
186719	8	415379	7	NULL	NULL	0	NULL	ovulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the mechanism of action of AGT-2 , we used a bovine granulosa cell model in which luteinizing hormone ( LH ) increased the expression of genes essential for ovulation in a time - and dose-dependent manner .
	manualset3
186720	9	415379	7	NULL	NULL	0	NULL	time-dependent manner	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the mechanism of action of AGT-2 , we used a bovine granulosa cell model in which luteinizing hormone ( LH ) increased the expression of genes essential for ovulation in a time - and dose-dependent manner .
	manualset3
186721	10	415379	7	NULL	NULL	0	NULL	dose-dependent manner	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the mechanism of action of AGT-2 , we used a bovine granulosa cell model in which luteinizing hormone ( LH ) increased the expression of genes essential for ovulation in a time - and dose-dependent manner .
	manualset3
186722	1	415380	7	NULL	NULL	0	NULL	molecular basis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the molecular basis for the different action of IL-2 and PSK , we investigated the upstream effects generated in human NKL cells by IL-2 and PSK on protein kinase C ( PKC ) isoenzymes and mitogen-activated protein kinases ( MAPK ) .
	manualset3
186723	2	415380	7	NULL	NULL	0	NULL	different action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the molecular basis for the different action of IL-2 and PSK , we investigated the upstream effects generated in human NKL cells by IL-2 and PSK on protein kinase C ( PKC ) isoenzymes and mitogen-activated protein kinases ( MAPK ) .
	manualset3
186724	3	415380	7	NULL	NULL	0	NULL	IL-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the molecular basis for the different action of IL-2 and PSK , we investigated the upstream effects generated in human NKL cells by IL-2 and PSK on protein kinase C ( PKC ) isoenzymes and mitogen-activated protein kinases ( MAPK ) .
	manualset3
186725	4	415380	7	NULL	NULL	0	NULL	PSK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the molecular basis for the different action of IL-2 and PSK , we investigated the upstream effects generated in human NKL cells by IL-2 and PSK on protein kinase C ( PKC ) isoenzymes and mitogen-activated protein kinases ( MAPK ) .
	manualset3
186726	5	415380	7	NULL	NULL	0	NULL	upstream effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the molecular basis for the different action of IL-2 and PSK , we investigated the upstream effects generated in human NKL cells by IL-2 and PSK on protein kinase C ( PKC ) isoenzymes and mitogen-activated protein kinases ( MAPK ) .
	manualset3
186727	6	415380	7	NULL	NULL	0	NULL	human NKL cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the molecular basis for the different action of IL-2 and PSK , we investigated the upstream effects generated in human NKL cells by IL-2 and PSK on protein kinase C ( PKC ) isoenzymes and mitogen-activated protein kinases ( MAPK ) .
	manualset3
186728	7	415380	7	NULL	NULL	0	NULL	 IL-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the molecular basis for the different action of IL-2 and PSK , we investigated the upstream effects generated in human NKL cells by IL-2 and PSK on protein kinase C ( PKC ) isoenzymes and mitogen-activated protein kinases ( MAPK ) .
	manualset3
186729	8	415380	7	NULL	NULL	0	NULL	PSK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the molecular basis for the different action of IL-2 and PSK , we investigated the upstream effects generated in human NKL cells by IL-2 and PSK on protein kinase C ( PKC ) isoenzymes and mitogen-activated protein kinases ( MAPK ) .
	manualset3
186730	9	415380	7	NULL	NULL	0	NULL	protein kinase C ( PKC ) isoenzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the molecular basis for the different action of IL-2 and PSK , we investigated the upstream effects generated in human NKL cells by IL-2 and PSK on protein kinase C ( PKC ) isoenzymes and mitogen-activated protein kinases ( MAPK ) .
	manualset3
186731	10	415380	7	NULL	NULL	0	NULL	mitogen-activated protein kinases ( MAPK ) 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the molecular basis for the different action of IL-2 and PSK , we investigated the upstream effects generated in human NKL cells by IL-2 and PSK on protein kinase C ( PKC ) isoenzymes and mitogen-activated protein kinases ( MAPK ) .
	manualset3
186732	1	415381	7	NULL	NULL	0	NULL	prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the prevalence of significant carotid artery disease in Hispanic patients with diabetes presenting with limb-threatening ischemia and to identify factors predictive of occurrence , we conducted a year-long prospective study of 92 consecutive patients undergoing infrainguinal bypass for limb salvage at The University of Texas Health Science Center in San Antonio .
	manualset3
186733	2	415381	7	NULL	NULL	0	NULL	carotid artery disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the prevalence of significant carotid artery disease in Hispanic patients with diabetes presenting with limb-threatening ischemia and to identify factors predictive of occurrence , we conducted a year-long prospective study of 92 consecutive patients undergoing infrainguinal bypass for limb salvage at The University of Texas Health Science Center in San Antonio .
	manualset3
186734	3	415381	7	NULL	NULL	0	NULL	Hispanic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the prevalence of significant carotid artery disease in Hispanic patients with diabetes presenting with limb-threatening ischemia and to identify factors predictive of occurrence , we conducted a year-long prospective study of 92 consecutive patients undergoing infrainguinal bypass for limb salvage at The University of Texas Health Science Center in San Antonio .
	manualset3
186735	4	415381	7	NULL	NULL	0	NULL	diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the prevalence of significant carotid artery disease in Hispanic patients with diabetes presenting with limb-threatening ischemia and to identify factors predictive of occurrence , we conducted a year-long prospective study of 92 consecutive patients undergoing infrainguinal bypass for limb salvage at The University of Texas Health Science Center in San Antonio .
	manualset3
186736	5	415381	7	NULL	NULL	0	NULL	limb-threatening ischemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the prevalence of significant carotid artery disease in Hispanic patients with diabetes presenting with limb-threatening ischemia and to identify factors predictive of occurrence , we conducted a year-long prospective study of 92 consecutive patients undergoing infrainguinal bypass for limb salvage at The University of Texas Health Science Center in San Antonio .
	manualset3
186737	6	415381	7	NULL	NULL	0	NULL	factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the prevalence of significant carotid artery disease in Hispanic patients with diabetes presenting with limb-threatening ischemia and to identify factors predictive of occurrence , we conducted a year-long prospective study of 92 consecutive patients undergoing infrainguinal bypass for limb salvage at The University of Texas Health Science Center in San Antonio .
	manualset3
186738	7	415381	7	NULL	NULL	0	NULL	predictive of occurrence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the prevalence of significant carotid artery disease in Hispanic patients with diabetes presenting with limb-threatening ischemia and to identify factors predictive of occurrence , we conducted a year-long prospective study of 92 consecutive patients undergoing infrainguinal bypass for limb salvage at The University of Texas Health Science Center in San Antonio .
	manualset3
186739	8	415381	7	NULL	NULL	0	NULL	year-long prospective study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the prevalence of significant carotid artery disease in Hispanic patients with diabetes presenting with limb-threatening ischemia and to identify factors predictive of occurrence , we conducted a year-long prospective study of 92 consecutive patients undergoing infrainguinal bypass for limb salvage at The University of Texas Health Science Center in San Antonio .
	manualset3
186740	9	415381	7	NULL	NULL	0	NULL	 92	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the prevalence of significant carotid artery disease in Hispanic patients with diabetes presenting with limb-threatening ischemia and to identify factors predictive of occurrence , we conducted a year-long prospective study of 92 consecutive patients undergoing infrainguinal bypass for limb salvage at The University of Texas Health Science Center in San Antonio .
	manualset3
186741	10	415381	7	NULL	NULL	0	NULL	consecutive patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the prevalence of significant carotid artery disease in Hispanic patients with diabetes presenting with limb-threatening ischemia and to identify factors predictive of occurrence , we conducted a year-long prospective study of 92 consecutive patients undergoing infrainguinal bypass for limb salvage at The University of Texas Health Science Center in San Antonio .
	manualset3
186742	11	415381	7	NULL	NULL	0	NULL	infrainguinal bypass 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the prevalence of significant carotid artery disease in Hispanic patients with diabetes presenting with limb-threatening ischemia and to identify factors predictive of occurrence , we conducted a year-long prospective study of 92 consecutive patients undergoing infrainguinal bypass for limb salvage at The University of Texas Health Science Center in San Antonio .
	manualset3
186743	12	415381	7	NULL	NULL	0	NULL	 limb salvage	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the prevalence of significant carotid artery disease in Hispanic patients with diabetes presenting with limb-threatening ischemia and to identify factors predictive of occurrence , we conducted a year-long prospective study of 92 consecutive patients undergoing infrainguinal bypass for limb salvage at The University of Texas Health Science Center in San Antonio .
	manualset3
186744	13	415381	7	NULL	NULL	0	NULL	University of Texas Health Science Center	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the prevalence of significant carotid artery disease in Hispanic patients with diabetes presenting with limb-threatening ischemia and to identify factors predictive of occurrence , we conducted a year-long prospective study of 92 consecutive patients undergoing infrainguinal bypass for limb salvage at The University of Texas Health Science Center in San Antonio .
	manualset3
186745	14	415381	7	NULL	NULL	0	NULL	San Antonio	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the prevalence of significant carotid artery disease in Hispanic patients with diabetes presenting with limb-threatening ischemia and to identify factors predictive of occurrence , we conducted a year-long prospective study of 92 consecutive patients undergoing infrainguinal bypass for limb salvage at The University of Texas Health Science Center in San Antonio .
	manualset3
186746	1	415382	7	NULL	NULL	0	NULL	relative analgesic efficacy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the relative analgesic efficacy of ibuprofen 400 mg and acetaminophen 1000 mg , we conducted a single-dose , double-blind , placebo-controlled , randomized clinical trial using a standard assay for analgesic agents , the dental pain model .
	manualset3
186747	2	415382	7	NULL	NULL	0	NULL	ibuprofen 400 mg 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the relative analgesic efficacy of ibuprofen 400 mg and acetaminophen 1000 mg , we conducted a single-dose , double-blind , placebo-controlled , randomized clinical trial using a standard assay for analgesic agents , the dental pain model .
	manualset3
186748	3	415382	7	NULL	NULL	0	NULL	acetaminophen 1000 mg	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the relative analgesic efficacy of ibuprofen 400 mg and acetaminophen 1000 mg , we conducted a single-dose , double-blind , placebo-controlled , randomized clinical trial using a standard assay for analgesic agents , the dental pain model .
	manualset3
186749	4	415382	7	NULL	NULL	0	NULL	single-dose clinical trial	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the relative analgesic efficacy of ibuprofen 400 mg and acetaminophen 1000 mg , we conducted a single-dose , double-blind , placebo-controlled , randomized clinical trial using a standard assay for analgesic agents , the dental pain model .
	manualset3
186750	5	415382	7	NULL	NULL	0	NULL	double-blind clinical trial	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the relative analgesic efficacy of ibuprofen 400 mg and acetaminophen 1000 mg , we conducted a single-dose , double-blind , placebo-controlled , randomized clinical trial using a standard assay for analgesic agents , the dental pain model .
	manualset3
186751	6	415382	7	NULL	NULL	0	NULL	placebo-controlled clinical trial	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the relative analgesic efficacy of ibuprofen 400 mg and acetaminophen 1000 mg , we conducted a single-dose , double-blind , placebo-controlled , randomized clinical trial using a standard assay for analgesic agents , the dental pain model .
	manualset3
186752	7	415382	7	NULL	NULL	0	NULL	randomized clinical trial	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the relative analgesic efficacy of ibuprofen 400 mg and acetaminophen 1000 mg , we conducted a single-dose , double-blind , placebo-controlled , randomized clinical trial using a standard assay for analgesic agents , the dental pain model .
	manualset3
186753	8	415382	7	NULL	NULL	0	NULL	standard assay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the relative analgesic efficacy of ibuprofen 400 mg and acetaminophen 1000 mg , we conducted a single-dose , double-blind , placebo-controlled , randomized clinical trial using a standard assay for analgesic agents , the dental pain model .
	manualset3
186754	9	415382	7	NULL	NULL	0	NULL	analgesic agents	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the relative analgesic efficacy of ibuprofen 400 mg and acetaminophen 1000 mg , we conducted a single-dose , double-blind , placebo-controlled , randomized clinical trial using a standard assay for analgesic agents , the dental pain model .
	manualset3
186755	10	415382	7	NULL	NULL	0	NULL	dental pain model 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the relative analgesic efficacy of ibuprofen 400 mg and acetaminophen 1000 mg , we conducted a single-dose , double-blind , placebo-controlled , randomized clinical trial using a standard assay for analgesic agents , the dental pain model .
	manualset3
186756	1	415383	7	NULL	NULL	0	NULL	 role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the role of calcium in these endothelin-induced contractions , the effects of diltiazem and nitrendipine were examined .
	manualset3
186757	2	415383	7	NULL	NULL	0	NULL	 calcium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the role of calcium in these endothelin-induced contractions , the effects of diltiazem and nitrendipine were examined .
	manualset3
186758	3	415383	7	NULL	NULL	0	NULL	endothelin-induced contractions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the role of calcium in these endothelin-induced contractions , the effects of diltiazem and nitrendipine were examined .
	manualset3
186759	4	415383	7	NULL	NULL	0	NULL	effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the role of calcium in these endothelin-induced contractions , the effects of diltiazem and nitrendipine were examined .
	manualset3
186760	5	415383	7	NULL	NULL	0	NULL	diltiazem	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the role of calcium in these endothelin-induced contractions , the effects of diltiazem and nitrendipine were examined .
	manualset3
186761	6	415383	7	NULL	NULL	0	NULL	nitrendipine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine the role of calcium in these endothelin-induced contractions , the effects of diltiazem and nitrendipine were examined .
	manualset3
186762	1	415384	7	NULL	NULL	0	NULL	activated Akt 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether activated Akt is required to prevent E1A-mediated apoptosis , ip 1-E1A-Axl cells were treated with the phosphatidylinositol-3 ' - OH kinase inhibitor wortmannin or transfected with a dominant negative Akt mutant .
	manualset3
186763	2	415384	7	NULL	NULL	0	NULL	E1A-mediated apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether activated Akt is required to prevent E1A-mediated apoptosis , ip 1-E1A-Axl cells were treated with the phosphatidylinositol-3 ' - OH kinase inhibitor wortmannin or transfected with a dominant negative Akt mutant .
	manualset3
186764	3	415384	7	NULL	NULL	0	NULL	ip 1-E1A-Axl cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether activated Akt is required to prevent E1A-mediated apoptosis , ip 1-E1A-Axl cells were treated with the phosphatidylinositol-3 ' - OH kinase inhibitor wortmannin or transfected with a dominant negative Akt mutant .
	manualset3
186765	4	415384	7	NULL	NULL	0	NULL	phosphatidylinositol-3 ' - OH kinase inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether activated Akt is required to prevent E1A-mediated apoptosis , ip 1-E1A-Axl cells were treated with the phosphatidylinositol-3 ' - OH kinase inhibitor wortmannin or transfected with a dominant negative Akt mutant .
	manualset3
186766	5	415384	7	NULL	NULL	0	NULL	wortmannin 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether activated Akt is required to prevent E1A-mediated apoptosis , ip 1-E1A-Axl cells were treated with the phosphatidylinositol-3 ' - OH kinase inhibitor wortmannin or transfected with a dominant negative Akt mutant .
	manualset3
186767	6	415384	7	NULL	NULL	0	NULL	dominant negative Akt mutant	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether activated Akt is required to prevent E1A-mediated apoptosis , ip 1-E1A-Axl cells were treated with the phosphatidylinositol-3 ' - OH kinase inhibitor wortmannin or transfected with a dominant negative Akt mutant .
	manualset3
186768	1	415385	7	NULL	NULL	0	NULL	 suspected risk factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjustment for suspected risk factors of UC , the higher indicators of urinary total arsenic levels , percentage of inorganic arsenic , percentage of MMA ( V ) , and primary methylation index were associated with increased risk of UC .
	manualset3
186769	2	415385	7	NULL	NULL	0	NULL	UC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjustment for suspected risk factors of UC , the higher indicators of urinary total arsenic levels , percentage of inorganic arsenic , percentage of MMA ( V ) , and primary methylation index were associated with increased risk of UC .
	manualset3
186770	3	415385	7	NULL	NULL	0	NULL	higher indicators	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjustment for suspected risk factors of UC , the higher indicators of urinary total arsenic levels , percentage of inorganic arsenic , percentage of MMA ( V ) , and primary methylation index were associated with increased risk of UC .
	manualset3
186771	4	415385	7	NULL	NULL	0	NULL	urinary total arsenic levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjustment for suspected risk factors of UC , the higher indicators of urinary total arsenic levels , percentage of inorganic arsenic , percentage of MMA ( V ) , and primary methylation index were associated with increased risk of UC .
	manualset3
186772	5	415385	7	NULL	NULL	0	NULL	percentage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjustment for suspected risk factors of UC , the higher indicators of urinary total arsenic levels , percentage of inorganic arsenic , percentage of MMA ( V ) , and primary methylation index were associated with increased risk of UC .
	manualset3
186773	6	415385	7	NULL	NULL	0	NULL	 inorganic arsenic 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjustment for suspected risk factors of UC , the higher indicators of urinary total arsenic levels , percentage of inorganic arsenic , percentage of MMA ( V ) , and primary methylation index were associated with increased risk of UC .
	manualset3
186774	7	415385	7	NULL	NULL	0	NULL	percentage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjustment for suspected risk factors of UC , the higher indicators of urinary total arsenic levels , percentage of inorganic arsenic , percentage of MMA ( V ) , and primary methylation index were associated with increased risk of UC .
	manualset3
186775	8	415385	7	NULL	NULL	0	NULL	MMA ( V )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjustment for suspected risk factors of UC , the higher indicators of urinary total arsenic levels , percentage of inorganic arsenic , percentage of MMA ( V ) , and primary methylation index were associated with increased risk of UC .
	manualset3
186776	9	415385	7	NULL	NULL	0	NULL	primary methylation index	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjustment for suspected risk factors of UC , the higher indicators of urinary total arsenic levels , percentage of inorganic arsenic , percentage of MMA ( V ) , and primary methylation index were associated with increased risk of UC .
	manualset3
186777	10	415385	7	NULL	NULL	NULL	NULL	increased risk	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After adjustment for suspected risk factors of UC , the higher indicators of urinary total arsenic levels , percentage of inorganic arsenic , percentage of MMA ( V ) , and primary methylation index were associated with increased risk of UC .
	manualset3
186778	11	415385	7	NULL	NULL	0	NULL	UC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjustment for suspected risk factors of UC , the higher indicators of urinary total arsenic levels , percentage of inorganic arsenic , percentage of MMA ( V ) , and primary methylation index were associated with increased risk of UC .
	manualset3
189774	12	415385	7	NULL	NULL	0	NULL	adjustment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjustment for suspected risk factors of UC , the higher indicators of urinary total arsenic levels , percentage of inorganic arsenic , percentage of MMA ( V ) , and primary methylation index were associated with increased risk of UC .
	manualset3
186779	1	415386	7	NULL	NULL	0	NULL	cancer procoagulant	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether cancer procoagulant was unique to the malignant state , procoagulant activity was assayed in extracts of normal and malignant tissue and serum-free medium from normal and transformed fibroblasts .
	manualset3
186780	2	415386	7	NULL	NULL	0	NULL	malignant state	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether cancer procoagulant was unique to the malignant state , procoagulant activity was assayed in extracts of normal and malignant tissue and serum-free medium from normal and transformed fibroblasts .
	manualset3
186781	3	415386	7	NULL	NULL	0	NULL	procoagulant activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether cancer procoagulant was unique to the malignant state , procoagulant activity was assayed in extracts of normal and malignant tissue and serum-free medium from normal and transformed fibroblasts .
	manualset3
186782	4	415386	7	NULL	NULL	0	NULL	extracts	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether cancer procoagulant was unique to the malignant state , procoagulant activity was assayed in extracts of normal and malignant tissue and serum-free medium from normal and transformed fibroblasts .
	manualset3
186783	5	415386	7	NULL	NULL	0	NULL	normal tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether cancer procoagulant was unique to the malignant state , procoagulant activity was assayed in extracts of normal and malignant tissue and serum-free medium from normal and transformed fibroblasts .
	manualset3
186784	6	415386	7	NULL	NULL	0	NULL	 malignant tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether cancer procoagulant was unique to the malignant state , procoagulant activity was assayed in extracts of normal and malignant tissue and serum-free medium from normal and transformed fibroblasts .
	manualset3
186785	7	415386	7	NULL	NULL	0	NULL	serum-free medium	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether cancer procoagulant was unique to the malignant state , procoagulant activity was assayed in extracts of normal and malignant tissue and serum-free medium from normal and transformed fibroblasts .
	manualset3
186786	8	415386	7	NULL	NULL	0	NULL	normal fibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether cancer procoagulant was unique to the malignant state , procoagulant activity was assayed in extracts of normal and malignant tissue and serum-free medium from normal and transformed fibroblasts .
	manualset3
186787	9	415386	7	NULL	NULL	0	NULL	transformed fibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether cancer procoagulant was unique to the malignant state , procoagulant activity was assayed in extracts of normal and malignant tissue and serum-free medium from normal and transformed fibroblasts .
	manualset3
186788	1	415387	7	NULL	NULL	0	NULL	constitutive activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether constitutive activity of SFK per se is sufficient to induce tumorigenesis in vivo , we have generated a mouse model with a keratinocyte-restricted deletion of the SFK-negative regulator csk ( Csk-K5 mice ) .
	manualset3
186789	2	415387	7	NULL	NULL	0	NULL	SFK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether constitutive activity of SFK per se is sufficient to induce tumorigenesis in vivo , we have generated a mouse model with a keratinocyte-restricted deletion of the SFK-negative regulator csk ( Csk-K5 mice ) .
	manualset3
186790	3	415387	7	NULL	NULL	0	NULL	tumorigenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether constitutive activity of SFK per se is sufficient to induce tumorigenesis in vivo , we have generated a mouse model with a keratinocyte-restricted deletion of the SFK-negative regulator csk ( Csk-K5 mice ) .
	manualset3
186791	4	415387	7	NULL	NULL	0	NULL	mouse model	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether constitutive activity of SFK per se is sufficient to induce tumorigenesis in vivo , we have generated a mouse model with a keratinocyte-restricted deletion of the SFK-negative regulator csk ( Csk-K5 mice ) .
	manualset3
186792	5	415387	7	NULL	NULL	0	NULL	keratinocyte-restricted deletion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether constitutive activity of SFK per se is sufficient to induce tumorigenesis in vivo , we have generated a mouse model with a keratinocyte-restricted deletion of the SFK-negative regulator csk ( Csk-K5 mice ) .
	manualset3
186793	6	415387	7	NULL	NULL	0	NULL	SFK-negative regulator csk ( Csk-K5 mice ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether constitutive activity of SFK per se is sufficient to induce tumorigenesis in vivo , we have generated a mouse model with a keratinocyte-restricted deletion of the SFK-negative regulator csk ( Csk-K5 mice ) .
	manualset3
186794	1	415388	7	NULL	NULL	0	NULL	dobutamine stress echocardiography ( DSE )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether dobutamine stress echocardiography ( DSE ) provides prognostic information beyond that available from routine clinical data , we reviewed the outcome of 210 consecutive patients referred for DSE to evaluate chest pain , perioperative risk , and myocardial viability .
	manualset3
186795	2	415388	7	NULL	NULL	0	NULL	prognostic information	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether dobutamine stress echocardiography ( DSE ) provides prognostic information beyond that available from routine clinical data , we reviewed the outcome of 210 consecutive patients referred for DSE to evaluate chest pain , perioperative risk , and myocardial viability .
	manualset3
186796	3	415388	7	NULL	NULL	0	NULL	routine clinical data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether dobutamine stress echocardiography ( DSE ) provides prognostic information beyond that available from routine clinical data , we reviewed the outcome of 210 consecutive patients referred for DSE to evaluate chest pain , perioperative risk , and myocardial viability .
	manualset3
186797	4	415388	7	NULL	NULL	0	NULL	outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether dobutamine stress echocardiography ( DSE ) provides prognostic information beyond that available from routine clinical data , we reviewed the outcome of 210 consecutive patients referred for DSE to evaluate chest pain , perioperative risk , and myocardial viability .
	manualset3
186798	5	415388	7	NULL	NULL	0	NULL	210 consecutive patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether dobutamine stress echocardiography ( DSE ) provides prognostic information beyond that available from routine clinical data , we reviewed the outcome of 210 consecutive patients referred for DSE to evaluate chest pain , perioperative risk , and myocardial viability .
	manualset3
186799	6	415388	7	NULL	NULL	0	NULL	DSE	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether dobutamine stress echocardiography ( DSE ) provides prognostic information beyond that available from routine clinical data , we reviewed the outcome of 210 consecutive patients referred for DSE to evaluate chest pain , perioperative risk , and myocardial viability .
	manualset3
186800	7	415388	7	NULL	NULL	0	NULL	chest pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether dobutamine stress echocardiography ( DSE ) provides prognostic information beyond that available from routine clinical data , we reviewed the outcome of 210 consecutive patients referred for DSE to evaluate chest pain , perioperative risk , and myocardial viability .
	manualset3
186801	8	415388	7	NULL	NULL	0	NULL	 perioperative risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether dobutamine stress echocardiography ( DSE ) provides prognostic information beyond that available from routine clinical data , we reviewed the outcome of 210 consecutive patients referred for DSE to evaluate chest pain , perioperative risk , and myocardial viability .
	manualset3
186802	9	415388	7	NULL	NULL	0	NULL	myocardial viability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether dobutamine stress echocardiography ( DSE ) provides prognostic information beyond that available from routine clinical data , we reviewed the outcome of 210 consecutive patients referred for DSE to evaluate chest pain , perioperative risk , and myocardial viability .
	manualset3
186803	1	415389	7	NULL	NULL	0	NULL	enhancer activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether enhancer and IRE activities could be separated , we introduced three 10-base pair substitutions into the 30-bp region .
	manualset3
186804	2	415389	7	NULL	NULL	0	NULL	IRE activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether enhancer and IRE activities could be separated , we introduced three 10-base pair substitutions into the 30-bp region .
	manualset3
186805	3	415389	7	NULL	NULL	0	NULL	three 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether enhancer and IRE activities could be separated , we introduced three 10-base pair substitutions into the 30-bp region .
	manualset3
186806	4	415389	7	NULL	NULL	0	NULL	10-base pair substitutions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether enhancer and IRE activities could be separated , we introduced three 10-base pair substitutions into the 30-bp region .
	manualset3
186807	5	415389	7	NULL	NULL	0	NULL	30-bp region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether enhancer and IRE activities could be separated , we introduced three 10-base pair substitutions into the 30-bp region .
	manualset3
186808	1	415390	7	NULL	NULL	0	NULL	metastatic calcification 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186809	2	415390	7	NULL	NULL	0	NULL	neointima formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186810	3	415390	7	NULL	NULL	0	NULL	neointimal calcification	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186811	4	415390	7	NULL	NULL	0	NULL	advanced human atherosclerosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186812	5	415390	7	NULL	NULL	0	NULL	32	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186813	6	415390	7	NULL	NULL	0	NULL	giant Flemish rabbits	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186814	7	415390	7	NULL	NULL	0	NULL	weight 5.5 + / - 0.6 kg	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186815	8	415390	7	NULL	NULL	NULL	NULL	overstretch balloon injury	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186816	9	415390	7	NULL	NULL	0	NULL	bilateral iliac arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186817	10	415390	7	NULL	NULL	0	NULL	diet therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186818	11	415390	7	NULL	NULL	0	NULL	8 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186819	12	415390	7	NULL	NULL	0	NULL	high cholesterol 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186820	13	415390	7	NULL	NULL	0	NULL	2 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186821	14	415390	7	NULL	NULL	0	NULL	low calcium-vitamin D2 regimen	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186822	15	415390	7	NULL	NULL	0	NULL	250 mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186823	16	415390	7	NULL	NULL	0	NULL	 calcium carbonate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186824	17	415390	7	NULL	NULL	0	NULL	5 times weekly	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186825	18	415390	7	NULL	NULL	0	NULL	50 , 000 U	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186826	19	415390	7	NULL	NULL	0	NULL	calciferol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186827	20	415390	7	NULL	NULL	0	NULL	 3 times weekly	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186828	21	415390	7	NULL	NULL	0	NULL	group 1	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186829	22	415390	7	NULL	NULL	0	NULL	n = 5	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186830	23	415390	7	NULL	NULL	0	NULL	low cholesterol 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186831	24	415390	7	NULL	NULL	NULL	NULL	0.5 %	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186832	25	415390	7	NULL	NULL	0	NULL	high calcium-vitamin D2 regimen	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186833	26	415390	7	NULL	NULL	0	NULL	500 mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186834	27	415390	7	NULL	NULL	0	NULL	calcium carbonate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186835	28	415390	7	NULL	NULL	0	NULL	5 times weekly	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186836	29	415390	7	NULL	NULL	0	NULL	100 , 000 U	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186837	30	415390	7	NULL	NULL	0	NULL	calciferol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186838	31	415390	7	NULL	NULL	0	NULL	three times weekly	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186839	32	415390	7	NULL	NULL	0	NULL	group 2	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186840	33	415390	7	NULL	NULL	NULL	NULL	n = 19	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186841	34	415390	7	NULL	NULL	0	NULL	0 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186842	35	415390	7	NULL	NULL	0	NULL	high calcium-vitamin D2 regimen	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186843	36	415390	7	NULL	NULL	0	NULL	group 3	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186844	37	415390	7	NULL	NULL	0	NULL	 n = 8	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
189008	38	415390	7	NULL	NULL	0	NULL	cholesterol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether metastatic calcification during neointima formation can result in neointimal calcification that simulates advanced human atherosclerosis , 32 giant Flemish rabbits ( weight 5.5 + / - 0.6 kg ) underwent overstretch balloon injury of bilateral iliac arteries and received diet therapy for 8 weeks : high cholesterol ( 2 % ) and low calcium-vitamin D2 regimen ( 250 mg of calcium carbonate orally 5 times weekly and 50 , 000 U of calciferol intramuscularly 3 times weekly ; group 1 ; n = 5 ) ; low cholesterol ( 0.5 % ) and high calcium-vitamin D2 regimen ( 500 mg of calcium carbonate orally 5 times weekly and 100 , 000 U of calciferol intramuscularly three times weekly ; group 2 ; n = 19 ) ; or 0 % cholesterol and high calcium-vitamin D2 regimen ( group 3 ; n = 8 ) .
	manualset3
186845	1	415391	7	NULL	NULL	0	NULL	modification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether modification of conditioned reinstatement by BD1047 is selective for drug-directed behavior or reflects general suppressant effects on motivated behavior , BD1047 was tested also on reinstatement induced by stimuli conditioned to a natural reward , sweetened condensed milk ( SCM ) .
	manualset3
186846	2	415391	7	NULL	NULL	0	NULL	conditioned reinstatement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether modification of conditioned reinstatement by BD1047 is selective for drug-directed behavior or reflects general suppressant effects on motivated behavior , BD1047 was tested also on reinstatement induced by stimuli conditioned to a natural reward , sweetened condensed milk ( SCM ) .
	manualset3
186847	3	415391	7	NULL	NULL	0	NULL	BD1047	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether modification of conditioned reinstatement by BD1047 is selective for drug-directed behavior or reflects general suppressant effects on motivated behavior , BD1047 was tested also on reinstatement induced by stimuli conditioned to a natural reward , sweetened condensed milk ( SCM ) .
	manualset3
186848	4	415391	7	NULL	NULL	0	NULL	drug-directed behavior	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether modification of conditioned reinstatement by BD1047 is selective for drug-directed behavior or reflects general suppressant effects on motivated behavior , BD1047 was tested also on reinstatement induced by stimuli conditioned to a natural reward , sweetened condensed milk ( SCM ) .
	manualset3
186849	5	415391	7	NULL	NULL	0	NULL	general suppressant effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether modification of conditioned reinstatement by BD1047 is selective for drug-directed behavior or reflects general suppressant effects on motivated behavior , BD1047 was tested also on reinstatement induced by stimuli conditioned to a natural reward , sweetened condensed milk ( SCM ) .
	manualset3
186850	6	415391	7	NULL	NULL	0	NULL	motivated behavior	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether modification of conditioned reinstatement by BD1047 is selective for drug-directed behavior or reflects general suppressant effects on motivated behavior , BD1047 was tested also on reinstatement induced by stimuli conditioned to a natural reward , sweetened condensed milk ( SCM ) .
	manualset3
186851	7	415391	7	NULL	NULL	0	NULL	BD1047 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether modification of conditioned reinstatement by BD1047 is selective for drug-directed behavior or reflects general suppressant effects on motivated behavior , BD1047 was tested also on reinstatement induced by stimuli conditioned to a natural reward , sweetened condensed milk ( SCM ) .
	manualset3
186852	8	415391	7	NULL	NULL	0	NULL	reinstatement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether modification of conditioned reinstatement by BD1047 is selective for drug-directed behavior or reflects general suppressant effects on motivated behavior , BD1047 was tested also on reinstatement induced by stimuli conditioned to a natural reward , sweetened condensed milk ( SCM ) .
	manualset3
186853	9	415391	7	NULL	NULL	0	NULL	stimuli 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether modification of conditioned reinstatement by BD1047 is selective for drug-directed behavior or reflects general suppressant effects on motivated behavior , BD1047 was tested also on reinstatement induced by stimuli conditioned to a natural reward , sweetened condensed milk ( SCM ) .
	manualset3
186854	10	415391	7	NULL	NULL	0	NULL	natural reward	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether modification of conditioned reinstatement by BD1047 is selective for drug-directed behavior or reflects general suppressant effects on motivated behavior , BD1047 was tested also on reinstatement induced by stimuli conditioned to a natural reward , sweetened condensed milk ( SCM ) .
	manualset3
186855	11	415391	7	NULL	NULL	0	NULL	sweetened condensed milk ( SCM )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether modification of conditioned reinstatement by BD1047 is selective for drug-directed behavior or reflects general suppressant effects on motivated behavior , BD1047 was tested also on reinstatement induced by stimuli conditioned to a natural reward , sweetened condensed milk ( SCM ) .
	manualset3
186856	1	415392	7	NULL	NULL	0	NULL	mothers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether mothers with panic disorder with or without agoraphobia interacted differently with their children than normal control mothers , 86 mothers and their adolescents ( aged between 13 and 23 years ) were observed during a structured play situation .
	manualset3
186857	2	415392	7	NULL	NULL	0	NULL	panic disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether mothers with panic disorder with or without agoraphobia interacted differently with their children than normal control mothers , 86 mothers and their adolescents ( aged between 13 and 23 years ) were observed during a structured play situation .
	manualset3
186858	3	415392	7	NULL	NULL	0	NULL	agoraphobia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether mothers with panic disorder with or without agoraphobia interacted differently with their children than normal control mothers , 86 mothers and their adolescents ( aged between 13 and 23 years ) were observed during a structured play situation .
	manualset3
186859	4	415392	7	NULL	NULL	0	NULL	 children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether mothers with panic disorder with or without agoraphobia interacted differently with their children than normal control mothers , 86 mothers and their adolescents ( aged between 13 and 23 years ) were observed during a structured play situation .
	manualset3
186860	5	415392	7	NULL	NULL	0	NULL	normal control mothers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether mothers with panic disorder with or without agoraphobia interacted differently with their children than normal control mothers , 86 mothers and their adolescents ( aged between 13 and 23 years ) were observed during a structured play situation .
	manualset3
186861	6	415392	7	NULL	NULL	0	NULL	86 mothers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether mothers with panic disorder with or without agoraphobia interacted differently with their children than normal control mothers , 86 mothers and their adolescents ( aged between 13 and 23 years ) were observed during a structured play situation .
	manualset3
186862	7	415392	7	NULL	NULL	0	NULL	adolescents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether mothers with panic disorder with or without agoraphobia interacted differently with their children than normal control mothers , 86 mothers and their adolescents ( aged between 13 and 23 years ) were observed during a structured play situation .
	manualset3
186863	8	415392	7	NULL	NULL	0	NULL	13 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether mothers with panic disorder with or without agoraphobia interacted differently with their children than normal control mothers , 86 mothers and their adolescents ( aged between 13 and 23 years ) were observed during a structured play situation .
	manualset3
186864	9	415392	7	NULL	NULL	0	NULL	23 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether mothers with panic disorder with or without agoraphobia interacted differently with their children than normal control mothers , 86 mothers and their adolescents ( aged between 13 and 23 years ) were observed during a structured play situation .
	manualset3
186865	10	415392	7	NULL	NULL	0	NULL	structured play situation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether mothers with panic disorder with or without agoraphobia interacted differently with their children than normal control mothers , 86 mothers and their adolescents ( aged between 13 and 23 years ) were observed during a structured play situation .
	manualset3
186866	1	415393	7	NULL	NULL	0	NULL	selenite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether selenite has estrogen-like activities , the effects of this compound on estrogen receptor-alpha ( ER-alpha ) and other estrogen-regulated genes were measured in the human breast cancer cell line MCF-7 .
	manualset3
186867	2	415393	7	NULL	NULL	0	NULL	estrogen-like activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether selenite has estrogen-like activities , the effects of this compound on estrogen receptor-alpha ( ER-alpha ) and other estrogen-regulated genes were measured in the human breast cancer cell line MCF-7 .
	manualset3
186868	3	415393	7	NULL	NULL	0	NULL	compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether selenite has estrogen-like activities , the effects of this compound on estrogen receptor-alpha ( ER-alpha ) and other estrogen-regulated genes were measured in the human breast cancer cell line MCF-7 .
	manualset3
186869	4	415393	7	NULL	NULL	NULL	NULL	estrogen receptor-alpha ( ER-alpha )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To determine whether selenite has estrogen-like activities , the effects of this compound on estrogen receptor-alpha ( ER-alpha ) and other estrogen-regulated genes were measured in the human breast cancer cell line MCF-7 .
	manualset3
186870	5	415393	7	NULL	NULL	0	NULL	estrogen-regulated genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether selenite has estrogen-like activities , the effects of this compound on estrogen receptor-alpha ( ER-alpha ) and other estrogen-regulated genes were measured in the human breast cancer cell line MCF-7 .
	manualset3
186871	6	415393	7	NULL	NULL	0	NULL	human breast cancer cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether selenite has estrogen-like activities , the effects of this compound on estrogen receptor-alpha ( ER-alpha ) and other estrogen-regulated genes were measured in the human breast cancer cell line MCF-7 .
	manualset3
186872	7	415393	7	NULL	NULL	0	NULL	MCF-7	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether selenite has estrogen-like activities , the effects of this compound on estrogen receptor-alpha ( ER-alpha ) and other estrogen-regulated genes were measured in the human breast cancer cell line MCF-7 .
	manualset3
189009	8	415393	7	NULL	NULL	0	NULL	effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether selenite has estrogen-like activities , the effects of this compound on estrogen receptor-alpha ( ER-alpha ) and other estrogen-regulated genes were measured in the human breast cancer cell line MCF-7 .
	manualset3
186873	1	415394	7	NULL	NULL	0	NULL	 induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether the induction of stromelysin-2 expression by growth factors and cytokines might be important for wound healing , we analyzed the expression of this gene during the healing process of full-thickness excisional wounds in mice .
	manualset3
186874	2	415394	7	NULL	NULL	0	NULL	stromelysin-2 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether the induction of stromelysin-2 expression by growth factors and cytokines might be important for wound healing , we analyzed the expression of this gene during the healing process of full-thickness excisional wounds in mice .
	manualset3
186875	3	415394	7	NULL	NULL	0	NULL	growth factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether the induction of stromelysin-2 expression by growth factors and cytokines might be important for wound healing , we analyzed the expression of this gene during the healing process of full-thickness excisional wounds in mice .
	manualset3
186876	4	415394	7	NULL	NULL	0	NULL	cytokines 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether the induction of stromelysin-2 expression by growth factors and cytokines might be important for wound healing , we analyzed the expression of this gene during the healing process of full-thickness excisional wounds in mice .
	manualset3
186877	5	415394	7	NULL	NULL	0	NULL	wound healing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether the induction of stromelysin-2 expression by growth factors and cytokines might be important for wound healing , we analyzed the expression of this gene during the healing process of full-thickness excisional wounds in mice .
	manualset3
186878	6	415394	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether the induction of stromelysin-2 expression by growth factors and cytokines might be important for wound healing , we analyzed the expression of this gene during the healing process of full-thickness excisional wounds in mice .
	manualset3
186879	7	415394	7	NULL	NULL	0	NULL	gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether the induction of stromelysin-2 expression by growth factors and cytokines might be important for wound healing , we analyzed the expression of this gene during the healing process of full-thickness excisional wounds in mice .
	manualset3
186880	8	415394	7	NULL	NULL	0	NULL	healing process	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether the induction of stromelysin-2 expression by growth factors and cytokines might be important for wound healing , we analyzed the expression of this gene during the healing process of full-thickness excisional wounds in mice .
	manualset3
186881	9	415394	7	NULL	NULL	0	NULL	full-thickness excisional wounds	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether the induction of stromelysin-2 expression by growth factors and cytokines might be important for wound healing , we analyzed the expression of this gene during the healing process of full-thickness excisional wounds in mice .
	manualset3
186882	10	415394	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether the induction of stromelysin-2 expression by growth factors and cytokines might be important for wound healing , we analyzed the expression of this gene during the healing process of full-thickness excisional wounds in mice .
	manualset3
186883	1	415395	7	NULL	NULL	0	NULL	covariates	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjustment for these covariates ( P & lt ; or = 0.04 for all ) , findings in men for iK ( CC versus T : 85.8 versus 87.3 mmol/l ; P = 0.14 ) and iMg ( 1.91 versus 1.82 mmol/l ; P = 0.03 ) remained consistent .
	manualset3
186884	2	415395	7	NULL	NULL	0	NULL	P & lt 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjustment for these covariates ( P & lt ; or = 0.04 for all ) , findings in men for iK ( CC versus T : 85.8 versus 87.3 mmol/l ; P = 0.14 ) and iMg ( 1.91 versus 1.82 mmol/l ; P = 0.03 ) remained consistent .
	manualset3
186885	3	415395	7	NULL	NULL	0	NULL	0.04	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjustment for these covariates ( P & lt ; or = 0.04 for all ) , findings in men for iK ( CC versus T : 85.8 versus 87.3 mmol/l ; P = 0.14 ) and iMg ( 1.91 versus 1.82 mmol/l ; P = 0.03 ) remained consistent .
	manualset3
186886	4	415395	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjustment for these covariates ( P & lt ; or = 0.04 for all ) , findings in men for iK ( CC versus T : 85.8 versus 87.3 mmol/l ; P = 0.14 ) and iMg ( 1.91 versus 1.82 mmol/l ; P = 0.03 ) remained consistent .
	manualset3
186887	5	415395	7	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjustment for these covariates ( P & lt ; or = 0.04 for all ) , findings in men for iK ( CC versus T : 85.8 versus 87.3 mmol/l ; P = 0.14 ) and iMg ( 1.91 versus 1.82 mmol/l ; P = 0.03 ) remained consistent .
	manualset3
186888	6	415395	7	NULL	NULL	0	NULL	iK	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjustment for these covariates ( P & lt ; or = 0.04 for all ) , findings in men for iK ( CC versus T : 85.8 versus 87.3 mmol/l ; P = 0.14 ) and iMg ( 1.91 versus 1.82 mmol/l ; P = 0.03 ) remained consistent .
	manualset3
186889	7	415395	7	NULL	NULL	0	NULL	CC versus T	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjustment for these covariates ( P & lt ; or = 0.04 for all ) , findings in men for iK ( CC versus T : 85.8 versus 87.3 mmol/l ; P = 0.14 ) and iMg ( 1.91 versus 1.82 mmol/l ; P = 0.03 ) remained consistent .
	manualset3
186890	8	415395	7	NULL	NULL	0	NULL	85.8 versus 87.3 mmol/l 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjustment for these covariates ( P & lt ; or = 0.04 for all ) , findings in men for iK ( CC versus T : 85.8 versus 87.3 mmol/l ; P = 0.14 ) and iMg ( 1.91 versus 1.82 mmol/l ; P = 0.03 ) remained consistent .
	manualset3
186891	9	415395	7	NULL	NULL	0	NULL	P = 0.14	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjustment for these covariates ( P & lt ; or = 0.04 for all ) , findings in men for iK ( CC versus T : 85.8 versus 87.3 mmol/l ; P = 0.14 ) and iMg ( 1.91 versus 1.82 mmol/l ; P = 0.03 ) remained consistent .
	manualset3
186892	10	415395	7	NULL	NULL	0	NULL	iMg	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjustment for these covariates ( P & lt ; or = 0.04 for all ) , findings in men for iK ( CC versus T : 85.8 versus 87.3 mmol/l ; P = 0.14 ) and iMg ( 1.91 versus 1.82 mmol/l ; P = 0.03 ) remained consistent .
	manualset3
186893	11	415395	7	NULL	NULL	0	NULL	1.91 versus 1.82 mmol/l 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjustment for these covariates ( P & lt ; or = 0.04 for all ) , findings in men for iK ( CC versus T : 85.8 versus 87.3 mmol/l ; P = 0.14 ) and iMg ( 1.91 versus 1.82 mmol/l ; P = 0.03 ) remained consistent .
	manualset3
186894	12	415395	7	NULL	NULL	0	NULL	P = 0.03	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	After adjustment for these covariates ( P & lt ; or = 0.04 for all ) , findings in men for iK ( CC versus T : 85.8 versus 87.3 mmol/l ; P = 0.14 ) and iMg ( 1.91 versus 1.82 mmol/l ; P = 0.03 ) remained consistent .
	manualset3
186895	1	415396	7	NULL	NULL	0	NULL	synthesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether the synthesis of IGF-binding proteins ( BPs ) is also affected by protein nutrition , we assessed plasma concentration , tissue mRNA content and liver transcription rate of each BP after rats were fed either a 12 % casein or a protein-free diet for 1 week .
	manualset3
186896	2	415396	7	NULL	NULL	0	NULL	IGF-binding proteins ( BPs )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether the synthesis of IGF-binding proteins ( BPs ) is also affected by protein nutrition , we assessed plasma concentration , tissue mRNA content and liver transcription rate of each BP after rats were fed either a 12 % casein or a protein-free diet for 1 week .
	manualset3
186897	3	415396	7	NULL	NULL	0	NULL	protein nutrition	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether the synthesis of IGF-binding proteins ( BPs ) is also affected by protein nutrition , we assessed plasma concentration , tissue mRNA content and liver transcription rate of each BP after rats were fed either a 12 % casein or a protein-free diet for 1 week .
	manualset3
186898	4	415396	7	NULL	NULL	0	NULL	plasma concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether the synthesis of IGF-binding proteins ( BPs ) is also affected by protein nutrition , we assessed plasma concentration , tissue mRNA content and liver transcription rate of each BP after rats were fed either a 12 % casein or a protein-free diet for 1 week .
	manualset3
186899	5	415396	7	NULL	NULL	0	NULL	tissue mRNA content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether the synthesis of IGF-binding proteins ( BPs ) is also affected by protein nutrition , we assessed plasma concentration , tissue mRNA content and liver transcription rate of each BP after rats were fed either a 12 % casein or a protein-free diet for 1 week .
	manualset3
186900	6	415396	7	NULL	NULL	0	NULL	liver transcription rate 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether the synthesis of IGF-binding proteins ( BPs ) is also affected by protein nutrition , we assessed plasma concentration , tissue mRNA content and liver transcription rate of each BP after rats were fed either a 12 % casein or a protein-free diet for 1 week .
	manualset3
186901	7	415396	7	NULL	NULL	0	NULL	BP	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether the synthesis of IGF-binding proteins ( BPs ) is also affected by protein nutrition , we assessed plasma concentration , tissue mRNA content and liver transcription rate of each BP after rats were fed either a 12 % casein or a protein-free diet for 1 week .
	manualset3
186902	8	415396	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether the synthesis of IGF-binding proteins ( BPs ) is also affected by protein nutrition , we assessed plasma concentration , tissue mRNA content and liver transcription rate of each BP after rats were fed either a 12 % casein or a protein-free diet for 1 week .
	manualset3
186903	9	415396	7	NULL	NULL	0	NULL	12 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether the synthesis of IGF-binding proteins ( BPs ) is also affected by protein nutrition , we assessed plasma concentration , tissue mRNA content and liver transcription rate of each BP after rats were fed either a 12 % casein or a protein-free diet for 1 week .
	manualset3
186904	10	415396	7	NULL	NULL	0	NULL	casein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether the synthesis of IGF-binding proteins ( BPs ) is also affected by protein nutrition , we assessed plasma concentration , tissue mRNA content and liver transcription rate of each BP after rats were fed either a 12 % casein or a protein-free diet for 1 week .
	manualset3
186905	11	415396	7	NULL	NULL	0	NULL	protein-free diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether the synthesis of IGF-binding proteins ( BPs ) is also affected by protein nutrition , we assessed plasma concentration , tissue mRNA content and liver transcription rate of each BP after rats were fed either a 12 % casein or a protein-free diet for 1 week .
	manualset3
186906	12	415396	7	NULL	NULL	0	NULL	1 week	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether the synthesis of IGF-binding proteins ( BPs ) is also affected by protein nutrition , we assessed plasma concentration , tissue mRNA content and liver transcription rate of each BP after rats were fed either a 12 % casein or a protein-free diet for 1 week .
	manualset3
186907	1	415397	7	NULL	NULL	0	NULL	thromboxane	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether thromboxane or oxygen-derived free radicals , a byproduct in the cyclooxygenase pathway , mediate this effect , subepicardial coronary arterioles ( 103 + / - 21 mu ) from New Zealand White rabbits were studied in vitro in a pressurized ( 40 mm Hg ) , no-flow state using videomicroscopy .
	manualset3
186908	2	415397	7	NULL	NULL	0	NULL	oxygen-derived free radicals	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether thromboxane or oxygen-derived free radicals , a byproduct in the cyclooxygenase pathway , mediate this effect , subepicardial coronary arterioles ( 103 + / - 21 mu ) from New Zealand White rabbits were studied in vitro in a pressurized ( 40 mm Hg ) , no-flow state using videomicroscopy .
	manualset3
186909	3	415397	7	NULL	NULL	0	NULL	byproduct	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether thromboxane or oxygen-derived free radicals , a byproduct in the cyclooxygenase pathway , mediate this effect , subepicardial coronary arterioles ( 103 + / - 21 mu ) from New Zealand White rabbits were studied in vitro in a pressurized ( 40 mm Hg ) , no-flow state using videomicroscopy .
	manualset3
186910	4	415397	7	NULL	NULL	0	NULL	cyclooxygenase pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether thromboxane or oxygen-derived free radicals , a byproduct in the cyclooxygenase pathway , mediate this effect , subepicardial coronary arterioles ( 103 + / - 21 mu ) from New Zealand White rabbits were studied in vitro in a pressurized ( 40 mm Hg ) , no-flow state using videomicroscopy .
	manualset3
186911	5	415397	7	NULL	NULL	0	NULL	subepicardial coronary arterioles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether thromboxane or oxygen-derived free radicals , a byproduct in the cyclooxygenase pathway , mediate this effect , subepicardial coronary arterioles ( 103 + / - 21 mu ) from New Zealand White rabbits were studied in vitro in a pressurized ( 40 mm Hg ) , no-flow state using videomicroscopy .
	manualset3
186912	6	415397	7	NULL	NULL	0	NULL	 103 + / - 21 mu	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether thromboxane or oxygen-derived free radicals , a byproduct in the cyclooxygenase pathway , mediate this effect , subepicardial coronary arterioles ( 103 + / - 21 mu ) from New Zealand White rabbits were studied in vitro in a pressurized ( 40 mm Hg ) , no-flow state using videomicroscopy .
	manualset3
186913	7	415397	7	NULL	NULL	0	NULL	New Zealand White rabbits	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether thromboxane or oxygen-derived free radicals , a byproduct in the cyclooxygenase pathway , mediate this effect , subepicardial coronary arterioles ( 103 + / - 21 mu ) from New Zealand White rabbits were studied in vitro in a pressurized ( 40 mm Hg ) , no-flow state using videomicroscopy .
	manualset3
186914	8	415397	7	NULL	NULL	0	NULL	40 mm Hg	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether thromboxane or oxygen-derived free radicals , a byproduct in the cyclooxygenase pathway , mediate this effect , subepicardial coronary arterioles ( 103 + / - 21 mu ) from New Zealand White rabbits were studied in vitro in a pressurized ( 40 mm Hg ) , no-flow state using videomicroscopy .
	manualset3
186915	9	415397	7	NULL	NULL	0	NULL	no-flow state	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether thromboxane or oxygen-derived free radicals , a byproduct in the cyclooxygenase pathway , mediate this effect , subepicardial coronary arterioles ( 103 + / - 21 mu ) from New Zealand White rabbits were studied in vitro in a pressurized ( 40 mm Hg ) , no-flow state using videomicroscopy .
	manualset3
186916	10	415397	7	NULL	NULL	0	NULL	videomicroscopy	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether thromboxane or oxygen-derived free radicals , a byproduct in the cyclooxygenase pathway , mediate this effect , subepicardial coronary arterioles ( 103 + / - 21 mu ) from New Zealand White rabbits were studied in vitro in a pressurized ( 40 mm Hg ) , no-flow state using videomicroscopy .
	manualset3
186917	1	415398	7	NULL	NULL	NULL	NULL	understanding	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To develop a clear understanding of the biochemical mechanism of muscle degeneration and regeneration induced by a single dose of Notechis scutatus scutatus venom , we have correlated changes in the levels of a series of muscle structural proteins and proteolytic enzymes .
	manualset3
186918	2	415398	7	NULL	NULL	0	NULL	biochemical mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop a clear understanding of the biochemical mechanism of muscle degeneration and regeneration induced by a single dose of Notechis scutatus scutatus venom , we have correlated changes in the levels of a series of muscle structural proteins and proteolytic enzymes .
	manualset3
186919	3	415398	7	NULL	NULL	0	NULL	muscle degeneration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop a clear understanding of the biochemical mechanism of muscle degeneration and regeneration induced by a single dose of Notechis scutatus scutatus venom , we have correlated changes in the levels of a series of muscle structural proteins and proteolytic enzymes .
	manualset3
186920	4	415398	7	NULL	NULL	0	NULL	regeneration 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop a clear understanding of the biochemical mechanism of muscle degeneration and regeneration induced by a single dose of Notechis scutatus scutatus venom , we have correlated changes in the levels of a series of muscle structural proteins and proteolytic enzymes .
	manualset3
186921	5	415398	7	NULL	NULL	0	NULL	single dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop a clear understanding of the biochemical mechanism of muscle degeneration and regeneration induced by a single dose of Notechis scutatus scutatus venom , we have correlated changes in the levels of a series of muscle structural proteins and proteolytic enzymes .
	manualset3
186922	6	415398	7	NULL	NULL	NULL	NULL	Notechis scutatus scutatus venom	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To develop a clear understanding of the biochemical mechanism of muscle degeneration and regeneration induced by a single dose of Notechis scutatus scutatus venom , we have correlated changes in the levels of a series of muscle structural proteins and proteolytic enzymes .
	manualset3
186923	7	415398	7	NULL	NULL	0	NULL	levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop a clear understanding of the biochemical mechanism of muscle degeneration and regeneration induced by a single dose of Notechis scutatus scutatus venom , we have correlated changes in the levels of a series of muscle structural proteins and proteolytic enzymes .
	manualset3
186924	8	415398	7	NULL	NULL	0	NULL	series	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop a clear understanding of the biochemical mechanism of muscle degeneration and regeneration induced by a single dose of Notechis scutatus scutatus venom , we have correlated changes in the levels of a series of muscle structural proteins and proteolytic enzymes .
	manualset3
186925	9	415398	7	NULL	NULL	0	NULL	muscle structural proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop a clear understanding of the biochemical mechanism of muscle degeneration and regeneration induced by a single dose of Notechis scutatus scutatus venom , we have correlated changes in the levels of a series of muscle structural proteins and proteolytic enzymes .
	manualset3
186926	10	415398	7	NULL	NULL	0	NULL	proteolytic enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop a clear understanding of the biochemical mechanism of muscle degeneration and regeneration induced by a single dose of Notechis scutatus scutatus venom , we have correlated changes in the levels of a series of muscle structural proteins and proteolytic enzymes .
	manualset3
189010	11	415398	7	NULL	NULL	0	NULL	changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop a clear understanding of the biochemical mechanism of muscle degeneration and regeneration induced by a single dose of Notechis scutatus scutatus venom , we have correlated changes in the levels of a series of muscle structural proteins and proteolytic enzymes .
	manualset3
186927	1	415399	7	NULL	NULL	0	NULL	animal model	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop an animal model for experimental nasal hypersensitivity and hyperreactivity , guinea pigs were subjected to intermittent exposure to cold temperature ( intermittent cold stress , SART stress ) for 5 consecutive days .
	manualset3
186928	2	415399	7	NULL	NULL	0	NULL	experimental nasal hypersensitivity	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop an animal model for experimental nasal hypersensitivity and hyperreactivity , guinea pigs were subjected to intermittent exposure to cold temperature ( intermittent cold stress , SART stress ) for 5 consecutive days .
	manualset3
186930	3	415399	7	NULL	NULL	NULL	NULL	experimental nasal hyperreactivity	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To develop an animal model for experimental nasal hypersensitivity and hyperreactivity , guinea pigs were subjected to intermittent exposure to cold temperature ( intermittent cold stress , SART stress ) for 5 consecutive days .
	manualset3
186931	4	415399	7	NULL	NULL	0	NULL	 guinea pigs 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop an animal model for experimental nasal hypersensitivity and hyperreactivity , guinea pigs were subjected to intermittent exposure to cold temperature ( intermittent cold stress , SART stress ) for 5 consecutive days .
	manualset3
186932	5	415399	7	NULL	NULL	0	NULL	 intermittent exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop an animal model for experimental nasal hypersensitivity and hyperreactivity , guinea pigs were subjected to intermittent exposure to cold temperature ( intermittent cold stress , SART stress ) for 5 consecutive days .
	manualset3
186933	6	415399	7	NULL	NULL	0	NULL	cold temperature	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop an animal model for experimental nasal hypersensitivity and hyperreactivity , guinea pigs were subjected to intermittent exposure to cold temperature ( intermittent cold stress , SART stress ) for 5 consecutive days .
	manualset3
186934	7	415399	7	NULL	NULL	0	NULL	intermittent cold stress	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop an animal model for experimental nasal hypersensitivity and hyperreactivity , guinea pigs were subjected to intermittent exposure to cold temperature ( intermittent cold stress , SART stress ) for 5 consecutive days .
	manualset3
186935	8	415399	7	NULL	NULL	0	NULL	SART stress 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop an animal model for experimental nasal hypersensitivity and hyperreactivity , guinea pigs were subjected to intermittent exposure to cold temperature ( intermittent cold stress , SART stress ) for 5 consecutive days .
	manualset3
186936	9	415399	7	NULL	NULL	0	NULL	5	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop an animal model for experimental nasal hypersensitivity and hyperreactivity , guinea pigs were subjected to intermittent exposure to cold temperature ( intermittent cold stress , SART stress ) for 5 consecutive days .
	manualset3
186937	10	415399	7	NULL	NULL	0	NULL	consecutive days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop an animal model for experimental nasal hypersensitivity and hyperreactivity , guinea pigs were subjected to intermittent exposure to cold temperature ( intermittent cold stress , SART stress ) for 5 consecutive days .
	manualset3
186938	1	415400	7	NULL	NULL	0	NULL	effective agents	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop more effective agents , we synthesized several derivatives , named HS-1183 , HS-1199 and HS-1200 , based on the structure of UDCA and CDCA , and investigated them for anti-proliferative activity in Jurkat cells , a human leukemic T cell line .
	manualset3
186939	2	415400	7	NULL	NULL	0	NULL	several derivatives	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop more effective agents , we synthesized several derivatives , named HS-1183 , HS-1199 and HS-1200 , based on the structure of UDCA and CDCA , and investigated them for anti-proliferative activity in Jurkat cells , a human leukemic T cell line .
	manualset3
186940	3	415400	7	NULL	NULL	0	NULL	HS-1183	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop more effective agents , we synthesized several derivatives , named HS-1183 , HS-1199 and HS-1200 , based on the structure of UDCA and CDCA , and investigated them for anti-proliferative activity in Jurkat cells , a human leukemic T cell line .
	manualset3
186941	4	415400	7	NULL	NULL	0	NULL	HS-1199	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop more effective agents , we synthesized several derivatives , named HS-1183 , HS-1199 and HS-1200 , based on the structure of UDCA and CDCA , and investigated them for anti-proliferative activity in Jurkat cells , a human leukemic T cell line .
	manualset3
186942	5	415400	7	NULL	NULL	0	NULL	HS-1200 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop more effective agents , we synthesized several derivatives , named HS-1183 , HS-1199 and HS-1200 , based on the structure of UDCA and CDCA , and investigated them for anti-proliferative activity in Jurkat cells , a human leukemic T cell line .
	manualset3
186943	6	415400	7	NULL	NULL	0	NULL	structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop more effective agents , we synthesized several derivatives , named HS-1183 , HS-1199 and HS-1200 , based on the structure of UDCA and CDCA , and investigated them for anti-proliferative activity in Jurkat cells , a human leukemic T cell line .
	manualset3
186944	7	415400	7	NULL	NULL	0	NULL	UDCA	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop more effective agents , we synthesized several derivatives , named HS-1183 , HS-1199 and HS-1200 , based on the structure of UDCA and CDCA , and investigated them for anti-proliferative activity in Jurkat cells , a human leukemic T cell line .
	manualset3
186945	8	415400	7	NULL	NULL	0	NULL	CDCA	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop more effective agents , we synthesized several derivatives , named HS-1183 , HS-1199 and HS-1200 , based on the structure of UDCA and CDCA , and investigated them for anti-proliferative activity in Jurkat cells , a human leukemic T cell line .
	manualset3
186946	9	415400	7	NULL	NULL	0	NULL	anti-proliferative activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop more effective agents , we synthesized several derivatives , named HS-1183 , HS-1199 and HS-1200 , based on the structure of UDCA and CDCA , and investigated them for anti-proliferative activity in Jurkat cells , a human leukemic T cell line .
	manualset3
186947	10	415400	7	NULL	NULL	0	NULL	Jurkat cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop more effective agents , we synthesized several derivatives , named HS-1183 , HS-1199 and HS-1200 , based on the structure of UDCA and CDCA , and investigated them for anti-proliferative activity in Jurkat cells , a human leukemic T cell line .
	manualset3
186948	11	415400	7	NULL	NULL	0	NULL	human leukemic T cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop more effective agents , we synthesized several derivatives , named HS-1183 , HS-1199 and HS-1200 , based on the structure of UDCA and CDCA , and investigated them for anti-proliferative activity in Jurkat cells , a human leukemic T cell line .
	manualset3
186949	1	415401	7	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop more reliable diagnosis of scabies , specific IgE antibodies to a major scabies antigen recombinant Sar s 14.3 ( rSar s 14.3 ) were measured in 140 plasma samples from scabies-infested and control subject groups using dissociation-enhanced lanthanide fluorescent immunoassays ( DELFIA ) .
	manualset3
186950	2	415401	7	NULL	NULL	0	NULL	scabies	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop more reliable diagnosis of scabies , specific IgE antibodies to a major scabies antigen recombinant Sar s 14.3 ( rSar s 14.3 ) were measured in 140 plasma samples from scabies-infested and control subject groups using dissociation-enhanced lanthanide fluorescent immunoassays ( DELFIA ) .
	manualset3
186951	3	415401	7	NULL	NULL	0	NULL	IgE antibodies	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop more reliable diagnosis of scabies , specific IgE antibodies to a major scabies antigen recombinant Sar s 14.3 ( rSar s 14.3 ) were measured in 140 plasma samples from scabies-infested and control subject groups using dissociation-enhanced lanthanide fluorescent immunoassays ( DELFIA ) .
	manualset3
186952	4	415401	7	NULL	NULL	0	NULL	scabies antigen recombinant Sar s 14.3 ( rSar s 14.3 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop more reliable diagnosis of scabies , specific IgE antibodies to a major scabies antigen recombinant Sar s 14.3 ( rSar s 14.3 ) were measured in 140 plasma samples from scabies-infested and control subject groups using dissociation-enhanced lanthanide fluorescent immunoassays ( DELFIA ) .
	manualset3
186953	5	415401	7	NULL	NULL	0	NULL	140	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop more reliable diagnosis of scabies , specific IgE antibodies to a major scabies antigen recombinant Sar s 14.3 ( rSar s 14.3 ) were measured in 140 plasma samples from scabies-infested and control subject groups using dissociation-enhanced lanthanide fluorescent immunoassays ( DELFIA ) .
	manualset3
186954	6	415401	7	NULL	NULL	0	NULL	plasma samples	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop more reliable diagnosis of scabies , specific IgE antibodies to a major scabies antigen recombinant Sar s 14.3 ( rSar s 14.3 ) were measured in 140 plasma samples from scabies-infested and control subject groups using dissociation-enhanced lanthanide fluorescent immunoassays ( DELFIA ) .
	manualset3
186955	7	415401	7	NULL	NULL	0	NULL	scabies-infested groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop more reliable diagnosis of scabies , specific IgE antibodies to a major scabies antigen recombinant Sar s 14.3 ( rSar s 14.3 ) were measured in 140 plasma samples from scabies-infested and control subject groups using dissociation-enhanced lanthanide fluorescent immunoassays ( DELFIA ) .
	manualset3
186956	8	415401	7	NULL	NULL	0	NULL	control subject groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop more reliable diagnosis of scabies , specific IgE antibodies to a major scabies antigen recombinant Sar s 14.3 ( rSar s 14.3 ) were measured in 140 plasma samples from scabies-infested and control subject groups using dissociation-enhanced lanthanide fluorescent immunoassays ( DELFIA ) .
	manualset3
186957	9	415401	7	NULL	NULL	0	NULL	dissociation-enhanced lanthanide fluorescent immunoassays ( DELFIA )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To develop more reliable diagnosis of scabies , specific IgE antibodies to a major scabies antigen recombinant Sar s 14.3 ( rSar s 14.3 ) were measured in 140 plasma samples from scabies-infested and control subject groups using dissociation-enhanced lanthanide fluorescent immunoassays ( DELFIA ) .
	manualset3
186958	1	415402	7	NULL	NULL	0	NULL	donor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To distinguish donor and recipient cells , we analyzed variable numbers of tandem repeats ( VNTRs ) polymorphisms using a YNH-24 probe by Southern blot hybridization .
	manualset3
186959	2	415402	7	NULL	NULL	0	NULL	recipient cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To distinguish donor and recipient cells , we analyzed variable numbers of tandem repeats ( VNTRs ) polymorphisms using a YNH-24 probe by Southern blot hybridization .
	manualset3
186960	3	415402	7	NULL	NULL	NULL	NULL	variable numbers of tandem repeats ( VNTRs ) polymorphisms	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To distinguish donor and recipient cells , we analyzed variable numbers of tandem repeats ( VNTRs ) polymorphisms using a YNH-24 probe by Southern blot hybridization .
	manualset3
186961	4	415402	7	NULL	NULL	0	NULL	YNH-24 probe	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To distinguish donor and recipient cells , we analyzed variable numbers of tandem repeats ( VNTRs ) polymorphisms using a YNH-24 probe by Southern blot hybridization .
	manualset3
186962	5	415402	7	NULL	NULL	0	NULL	Southern blot hybridization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To distinguish donor and recipient cells , we analyzed variable numbers of tandem repeats ( VNTRs ) polymorphisms using a YNH-24 probe by Southern blot hybridization .
	manualset3
186963	1	415403	7	NULL	NULL	0	NULL	Computed tomographic localization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Computed tomographic localization of the uterus for optimization of primary combined radiotherapy of inoperable cervix cancer ) .
	manualset3
186964	2	415403	7	NULL	NULL	0	NULL	uterus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Computed tomographic localization of the uterus for optimization of primary combined radiotherapy of inoperable cervix cancer ) .
	manualset3
186965	3	415403	7	NULL	NULL	0	NULL	optimization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Computed tomographic localization of the uterus for optimization of primary combined radiotherapy of inoperable cervix cancer ) .
	manualset3
186966	4	415403	7	NULL	NULL	0	NULL	primary combined radiotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Computed tomographic localization of the uterus for optimization of primary combined radiotherapy of inoperable cervix cancer ) .
	manualset3
186967	5	415403	7	NULL	NULL	0	NULL	inoperable cervix cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Computed tomographic localization of the uterus for optimization of primary combined radiotherapy of inoperable cervix cancer ) .
	manualset3
186968	1	415404	7	NULL	NULL	0	NULL	recombinant canine adenovirus type 2 genome pPoly2-CAV2-deltaE3-Rgp bearing exogenous Rgp gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	To efficiently construct cloned recombinant canine adenovirus type 2 genome pPoly2-CAV2-deltaE3-Rgp bearing exogenous Rgp gene , The Rgp gene was first subcloned from the clone vector pMD18-T into the eukaryon expression vector pVAX1 .
	manualset3
186969	2	415404	7	NULL	NULL	0	NULL	Rgp gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	To efficiently construct cloned recombinant canine adenovirus type 2 genome pPoly2-CAV2-deltaE3-Rgp bearing exogenous Rgp gene , The Rgp gene was first subcloned from the clone vector pMD18-T into the eukaryon expression vector pVAX1 .
	manualset3
186970	3	415404	7	NULL	NULL	0	NULL	clone vector pMD18-T	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To efficiently construct cloned recombinant canine adenovirus type 2 genome pPoly2-CAV2-deltaE3-Rgp bearing exogenous Rgp gene , The Rgp gene was first subcloned from the clone vector pMD18-T into the eukaryon expression vector pVAX1 .
	manualset3
186971	4	415404	7	NULL	NULL	0	NULL	 eukaryon expression vector pVAX1	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To efficiently construct cloned recombinant canine adenovirus type 2 genome pPoly2-CAV2-deltaE3-Rgp bearing exogenous Rgp gene , The Rgp gene was first subcloned from the clone vector pMD18-T into the eukaryon expression vector pVAX1 .
	manualset3
186972	1	415405	7	NULL	NULL	0	NULL	influence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To eliminate the influence of motor processing prior to S2 , a button press on the side of the higher bar was held until perception of a response cue ( S3 ) .
	manualset3
186973	2	415405	7	NULL	NULL	0	NULL	motor processing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To eliminate the influence of motor processing prior to S2 , a button press on the side of the higher bar was held until perception of a response cue ( S3 ) .
	manualset3
186974	3	415405	7	NULL	NULL	NULL	NULL	S2	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To eliminate the influence of motor processing prior to S2 , a button press on the side of the higher bar was held until perception of a response cue ( S3 ) .
	manualset3
186975	4	415405	7	NULL	NULL	0	NULL	button	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To eliminate the influence of motor processing prior to S2 , a button press on the side of the higher bar was held until perception of a response cue ( S3 ) .
	manualset3
186976	5	415405	7	NULL	NULL	0	NULL	higher bar	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To eliminate the influence of motor processing prior to S2 , a button press on the side of the higher bar was held until perception of a response cue ( S3 ) .
	manualset3
186977	6	415405	7	NULL	NULL	0	NULL	perception	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To eliminate the influence of motor processing prior to S2 , a button press on the side of the higher bar was held until perception of a response cue ( S3 ) .
	manualset3
186978	7	415405	7	NULL	NULL	0	NULL	 response cue ( S3 )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To eliminate the influence of motor processing prior to S2 , a button press on the side of the higher bar was held until perception of a response cue ( S3 ) .
	manualset3
186979	1	415406	7	NULL	NULL	0	NULL	serious potential complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To eliminate the serious potential complications of inadvertent coil embolization to undesirable sites and to improve control of the coil throughout the procedure , a modified snare-assisted method with approach from the main pulmonary artery was developed .
	manualset3
186980	2	415406	7	NULL	NULL	0	NULL	inadvertent coil embolization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To eliminate the serious potential complications of inadvertent coil embolization to undesirable sites and to improve control of the coil throughout the procedure , a modified snare-assisted method with approach from the main pulmonary artery was developed .
	manualset3
186981	3	415406	7	NULL	NULL	0	NULL	undesirable sites	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To eliminate the serious potential complications of inadvertent coil embolization to undesirable sites and to improve control of the coil throughout the procedure , a modified snare-assisted method with approach from the main pulmonary artery was developed .
	manualset3
186982	4	415406	7	NULL	NULL	0	NULL	control 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To eliminate the serious potential complications of inadvertent coil embolization to undesirable sites and to improve control of the coil throughout the procedure , a modified snare-assisted method with approach from the main pulmonary artery was developed .
	manualset3
186983	5	415406	7	NULL	NULL	0	NULL	 coil	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	To eliminate the serious potential complications of inadvertent coil embolization to undesirable sites and to improve control of the coil throughout the procedure , a modified snare-assisted method with approach from the main pulmonary artery was developed .
	manualset3
186984	6	415406	7	NULL	NULL	0	NULL	procedure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To eliminate the serious potential complications of inadvertent coil embolization to undesirable sites and to improve control of the coil throughout the procedure , a modified snare-assisted method with approach from the main pulmonary artery was developed .
	manualset3
186985	7	415406	7	NULL	NULL	0	NULL	snare-assisted method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To eliminate the serious potential complications of inadvertent coil embolization to undesirable sites and to improve control of the coil throughout the procedure , a modified snare-assisted method with approach from the main pulmonary artery was developed .
	manualset3
186986	8	415406	7	NULL	NULL	0	NULL	approach	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To eliminate the serious potential complications of inadvertent coil embolization to undesirable sites and to improve control of the coil throughout the procedure , a modified snare-assisted method with approach from the main pulmonary artery was developed .
	manualset3
186987	9	415406	7	NULL	NULL	0	NULL	main pulmonary artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To eliminate the serious potential complications of inadvertent coil embolization to undesirable sites and to improve control of the coil throughout the procedure , a modified snare-assisted method with approach from the main pulmonary artery was developed .
	manualset3
187166	1	415407	7	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To elucidate its role in cancer development and as a potential imprinted tumor suppressor , we investigated the allele-specific expression of the human p73 gene in 28 cases of renal cell carcinoma and its imprinting status in fetal pancreatic and thymic tissues .
	manualset3
187169	2	415407	7	NULL	NULL	0	NULL	cancer development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To elucidate its role in cancer development and as a potential imprinted tumor suppressor , we investigated the allele-specific expression of the human p73 gene in 28 cases of renal cell carcinoma and its imprinting status in fetal pancreatic and thymic tissues .
	manualset3
187173	3	415407	7	NULL	NULL	0	NULL	tumor suppressor	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	To elucidate its role in cancer development and as a potential imprinted tumor suppressor , we investigated the allele-specific expression of the human p73 gene in 28 cases of renal cell carcinoma and its imprinting status in fetal pancreatic and thymic tissues .
	manualset3
187174	4	415407	7	NULL	NULL	0	NULL	allele-specific expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To elucidate its role in cancer development and as a potential imprinted tumor suppressor , we investigated the allele-specific expression of the human p73 gene in 28 cases of renal cell carcinoma and its imprinting status in fetal pancreatic and thymic tissues .
	manualset3
187175	5	415407	7	NULL	NULL	0	NULL	human p73 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	To elucidate its role in cancer development and as a potential imprinted tumor suppressor , we investigated the allele-specific expression of the human p73 gene in 28 cases of renal cell carcinoma and its imprinting status in fetal pancreatic and thymic tissues .
	manualset3
187176	6	415407	7	NULL	NULL	0	NULL	28 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To elucidate its role in cancer development and as a potential imprinted tumor suppressor , we investigated the allele-specific expression of the human p73 gene in 28 cases of renal cell carcinoma and its imprinting status in fetal pancreatic and thymic tissues .
	manualset3
187177	7	415407	7	NULL	NULL	0	NULL	renal cell carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To elucidate its role in cancer development and as a potential imprinted tumor suppressor , we investigated the allele-specific expression of the human p73 gene in 28 cases of renal cell carcinoma and its imprinting status in fetal pancreatic and thymic tissues .
	manualset3
187178	8	415407	7	NULL	NULL	0	NULL	 imprinting status	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To elucidate its role in cancer development and as a potential imprinted tumor suppressor , we investigated the allele-specific expression of the human p73 gene in 28 cases of renal cell carcinoma and its imprinting status in fetal pancreatic and thymic tissues .
	manualset3
187179	9	415407	7	NULL	NULL	0	NULL	fetal pancreatic tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	To elucidate its role in cancer development and as a potential imprinted tumor suppressor , we investigated the allele-specific expression of the human p73 gene in 28 cases of renal cell carcinoma and its imprinting status in fetal pancreatic and thymic tissues .
	manualset3
187181	10	415407	7	NULL	NULL	0	NULL	thymic tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	To elucidate its role in cancer development and as a potential imprinted tumor suppressor , we investigated the allele-specific expression of the human p73 gene in 28 cases of renal cell carcinoma and its imprinting status in fetal pancreatic and thymic tissues .
	manualset3
187188	1	415408	7	NULL	NULL	0	NULL	modulators	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To elucidate the modulators of net plasminogen activation on the cell surface , we have recently established an assay system .
	manualset3
187189	2	415408	7	NULL	NULL	0	NULL	net plasminogen activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To elucidate the modulators of net plasminogen activation on the cell surface , we have recently established an assay system .
	manualset3
187190	3	415408	7	NULL	NULL	0	NULL	cell surface	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	To elucidate the modulators of net plasminogen activation on the cell surface , we have recently established an assay system .
	manualset3
187191	4	415408	7	NULL	NULL	0	NULL	assay system	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To elucidate the modulators of net plasminogen activation on the cell surface , we have recently established an assay system .
	manualset3
187192	1	415409	7	NULL	NULL	0	NULL	 molecular nature	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To elucidate the molecular nature of the vacC locus , we cloned the vacC region from YSH6000 on a 1.8-kb SalI-BamHI DNA fragment .
	manualset3
187193	2	415409	7	NULL	NULL	0	NULL	vacC locus	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	To elucidate the molecular nature of the vacC locus , we cloned the vacC region from YSH6000 on a 1.8-kb SalI-BamHI DNA fragment .
	manualset3
187194	3	415409	7	NULL	NULL	0	NULL	vacC region	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	To elucidate the molecular nature of the vacC locus , we cloned the vacC region from YSH6000 on a 1.8-kb SalI-BamHI DNA fragment .
	manualset3
187195	4	415409	7	NULL	NULL	0	NULL	YSH6000	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To elucidate the molecular nature of the vacC locus , we cloned the vacC region from YSH6000 on a 1.8-kb SalI-BamHI DNA fragment .
	manualset3
187196	5	415409	7	NULL	NULL	0	NULL	1.8-kb SalI-BamHI DNA fragment	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To elucidate the molecular nature of the vacC locus , we cloned the vacC region from YSH6000 on a 1.8-kb SalI-BamHI DNA fragment .
	manualset3
187197	1	415410	7	NULL	NULL	0	NULL	 role 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To elucidate the role of mgcl-1 , we analyzed two mutant mouse lines that lacked mgcl-1 gene expression .
	manualset3
187198	2	415410	7	NULL	NULL	0	NULL	mgcl-1	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	To elucidate the role of mgcl-1 , we analyzed two mutant mouse lines that lacked mgcl-1 gene expression .
	manualset3
187199	3	415410	7	NULL	NULL	0	NULL	two mutant mouse lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To elucidate the role of mgcl-1 , we analyzed two mutant mouse lines that lacked mgcl-1 gene expression .
	manualset3
187200	4	415410	7	NULL	NULL	0	NULL	mgcl-1 gene expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To elucidate the role of mgcl-1 , we analyzed two mutant mouse lines that lacked mgcl-1 gene expression .
	manualset3
187201	1	415411	7	NULL	NULL	0	NULL	proper representation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To ensure proper representation , three examples of each brand of dental radiometer were used .
	manualset3
187202	2	415411	7	NULL	NULL	0	NULL	three examples	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To ensure proper representation , three examples of each brand of dental radiometer were used .
	manualset3
187203	3	415411	7	NULL	NULL	0	NULL	brand	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	To ensure proper representation , three examples of each brand of dental radiometer were used .
	manualset3
187204	4	415411	7	NULL	NULL	0	NULL	dental radiometer 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	To ensure proper representation , three examples of each brand of dental radiometer were used .
	manualset3
187205	1	415412	7	NULL	NULL	0	NULL	macular cone structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate macular cone structure in patients with X-linked retinoschisis ( XLRS ) caused by mutations in exon 6 of the RS1 gene .
	manualset3
187206	2	415412	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate macular cone structure in patients with X-linked retinoschisis ( XLRS ) caused by mutations in exon 6 of the RS1 gene .
	manualset3
187207	3	415412	7	NULL	NULL	0	NULL	X-linked retinoschisis ( XLRS )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate macular cone structure in patients with X-linked retinoschisis ( XLRS ) caused by mutations in exon 6 of the RS1 gene .
	manualset3
187208	4	415412	7	NULL	NULL	0	NULL	mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate macular cone structure in patients with X-linked retinoschisis ( XLRS ) caused by mutations in exon 6 of the RS1 gene .
	manualset3
187209	5	415412	7	NULL	NULL	0	NULL	 exon 6	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate macular cone structure in patients with X-linked retinoschisis ( XLRS ) caused by mutations in exon 6 of the RS1 gene .
	manualset3
187210	6	415412	7	NULL	NULL	0	NULL	RS1 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate macular cone structure in patients with X-linked retinoschisis ( XLRS ) caused by mutations in exon 6 of the RS1 gene .
	manualset3
187211	1	415413	7	NULL	NULL	0	NULL	age 65	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	After age 65 , rates of dementia tend to double every five years in developed countries and every seven in developing ones .
	manualset3
187212	2	415413	7	NULL	NULL	0	NULL	rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After age 65 , rates of dementia tend to double every five years in developed countries and every seven in developing ones .
	manualset3
187213	3	415413	7	NULL	NULL	0	NULL	dementia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	After age 65 , rates of dementia tend to double every five years in developed countries and every seven in developing ones .
	manualset3
187214	4	415413	7	NULL	NULL	0	NULL	five years	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	After age 65 , rates of dementia tend to double every five years in developed countries and every seven in developing ones .
	manualset3
187215	5	415413	7	NULL	NULL	0	NULL	developed countries	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	After age 65 , rates of dementia tend to double every five years in developed countries and every seven in developing ones .
	manualset3
187216	6	415413	7	NULL	NULL	0	NULL	seven	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After age 65 , rates of dementia tend to double every five years in developed countries and every seven in developing ones .
	manualset3
187217	7	415413	7	NULL	NULL	0	NULL	developing ones	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	After age 65 , rates of dementia tend to double every five years in developed countries and every seven in developing ones .
	manualset3
187218	1	415414	7	NULL	NULL	0	NULL	Merritt coils	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate our Merritt coils we solved the Biot-Savart law explicitly for ideal 3-coil and 4-coil Merritt systems and compared these theoretical EMFs with those of our systems .
	manualset3
187219	2	415414	7	NULL	NULL	0	NULL	Biot-Savart law	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate our Merritt coils we solved the Biot-Savart law explicitly for ideal 3-coil and 4-coil Merritt systems and compared these theoretical EMFs with those of our systems .
	manualset3
187220	3	415414	7	NULL	NULL	0	NULL	ideal 3-coil Merritt systems 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate our Merritt coils we solved the Biot-Savart law explicitly for ideal 3-coil and 4-coil Merritt systems and compared these theoretical EMFs with those of our systems .
	manualset3
187221	4	415414	7	NULL	NULL	0	NULL	4-coil Merritt systems	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate our Merritt coils we solved the Biot-Savart law explicitly for ideal 3-coil and 4-coil Merritt systems and compared these theoretical EMFs with those of our systems .
	manualset3
187222	5	415414	7	NULL	NULL	0	NULL	theoretical EMFs	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate our Merritt coils we solved the Biot-Savart law explicitly for ideal 3-coil and 4-coil Merritt systems and compared these theoretical EMFs with those of our systems .
	manualset3
187223	6	415414	7	NULL	NULL	0	NULL	systems	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate our Merritt coils we solved the Biot-Savart law explicitly for ideal 3-coil and 4-coil Merritt systems and compared these theoretical EMFs with those of our systems .
	manualset3
187224	1	415415	7	NULL	NULL	0	NULL	degree	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the degree of anthropogenic mercury pollution , Hg contents have been measured for box-core sediments sampled along three nearshore-offshore transects in the Strait of Sicily and well constrained for their mineralogy , bulk geochemistry and TOC % .
	manualset3
187225	2	415415	7	NULL	NULL	0	NULL	anthropogenic mercury pollution	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the degree of anthropogenic mercury pollution , Hg contents have been measured for box-core sediments sampled along three nearshore-offshore transects in the Strait of Sicily and well constrained for their mineralogy , bulk geochemistry and TOC % .
	manualset3
187226	3	415415	7	NULL	NULL	0	NULL	 Hg contents	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the degree of anthropogenic mercury pollution , Hg contents have been measured for box-core sediments sampled along three nearshore-offshore transects in the Strait of Sicily and well constrained for their mineralogy , bulk geochemistry and TOC % .
	manualset3
187227	4	415415	7	NULL	NULL	0	NULL	box-core sediments	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the degree of anthropogenic mercury pollution , Hg contents have been measured for box-core sediments sampled along three nearshore-offshore transects in the Strait of Sicily and well constrained for their mineralogy , bulk geochemistry and TOC % .
	manualset3
187228	5	415415	7	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the degree of anthropogenic mercury pollution , Hg contents have been measured for box-core sediments sampled along three nearshore-offshore transects in the Strait of Sicily and well constrained for their mineralogy , bulk geochemistry and TOC % .
	manualset3
187229	6	415415	7	NULL	NULL	0	NULL	nearshore-offshore transects	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the degree of anthropogenic mercury pollution , Hg contents have been measured for box-core sediments sampled along three nearshore-offshore transects in the Strait of Sicily and well constrained for their mineralogy , bulk geochemistry and TOC % .
	manualset3
187230	7	415415	7	NULL	NULL	0	NULL	Strait of Sicily 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the degree of anthropogenic mercury pollution , Hg contents have been measured for box-core sediments sampled along three nearshore-offshore transects in the Strait of Sicily and well constrained for their mineralogy , bulk geochemistry and TOC % .
	manualset3
187231	8	415415	7	NULL	NULL	0	NULL	 mineralogy	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the degree of anthropogenic mercury pollution , Hg contents have been measured for box-core sediments sampled along three nearshore-offshore transects in the Strait of Sicily and well constrained for their mineralogy , bulk geochemistry and TOC % .
	manualset3
187232	9	415415	7	NULL	NULL	0	NULL	bulk geochemistry	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the degree of anthropogenic mercury pollution , Hg contents have been measured for box-core sediments sampled along three nearshore-offshore transects in the Strait of Sicily and well constrained for their mineralogy , bulk geochemistry and TOC % .
	manualset3
187233	10	415415	7	NULL	NULL	0	NULL	TOC %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the degree of anthropogenic mercury pollution , Hg contents have been measured for box-core sediments sampled along three nearshore-offshore transects in the Strait of Sicily and well constrained for their mineralogy , bulk geochemistry and TOC % .
	manualset3
187234	1	415416	7	NULL	NULL	0	NULL	effect 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the effect of CD133 ( + ) cells ( endothelial progenitor cells ) on the hypoxia-induced suppression of axonal growth of cortical neurons and the destruction of blood vessels ( endothelial cells ) , we used anterograde axonal tracing and immunofluorescence in organ co-cultures of the cortex and the spinal cord from 3-day-old neonatal rats .
	manualset3
187235	2	415416	7	NULL	NULL	0	NULL	CD133 ( + ) cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the effect of CD133 ( + ) cells ( endothelial progenitor cells ) on the hypoxia-induced suppression of axonal growth of cortical neurons and the destruction of blood vessels ( endothelial cells ) , we used anterograde axonal tracing and immunofluorescence in organ co-cultures of the cortex and the spinal cord from 3-day-old neonatal rats .
	manualset3
187236	3	415416	7	NULL	NULL	0	NULL	endothelial progenitor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the effect of CD133 ( + ) cells ( endothelial progenitor cells ) on the hypoxia-induced suppression of axonal growth of cortical neurons and the destruction of blood vessels ( endothelial cells ) , we used anterograde axonal tracing and immunofluorescence in organ co-cultures of the cortex and the spinal cord from 3-day-old neonatal rats .
	manualset3
187237	4	415416	7	NULL	NULL	0	NULL	hypoxia-induced suppression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the effect of CD133 ( + ) cells ( endothelial progenitor cells ) on the hypoxia-induced suppression of axonal growth of cortical neurons and the destruction of blood vessels ( endothelial cells ) , we used anterograde axonal tracing and immunofluorescence in organ co-cultures of the cortex and the spinal cord from 3-day-old neonatal rats .
	manualset3
187238	5	415416	7	NULL	NULL	0	NULL	 axonal growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the effect of CD133 ( + ) cells ( endothelial progenitor cells ) on the hypoxia-induced suppression of axonal growth of cortical neurons and the destruction of blood vessels ( endothelial cells ) , we used anterograde axonal tracing and immunofluorescence in organ co-cultures of the cortex and the spinal cord from 3-day-old neonatal rats .
	manualset3
187239	6	415416	7	NULL	NULL	0	NULL	cortical neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the effect of CD133 ( + ) cells ( endothelial progenitor cells ) on the hypoxia-induced suppression of axonal growth of cortical neurons and the destruction of blood vessels ( endothelial cells ) , we used anterograde axonal tracing and immunofluorescence in organ co-cultures of the cortex and the spinal cord from 3-day-old neonatal rats .
	manualset3
187240	7	415416	7	NULL	NULL	0	NULL	destruction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the effect of CD133 ( + ) cells ( endothelial progenitor cells ) on the hypoxia-induced suppression of axonal growth of cortical neurons and the destruction of blood vessels ( endothelial cells ) , we used anterograde axonal tracing and immunofluorescence in organ co-cultures of the cortex and the spinal cord from 3-day-old neonatal rats .
	manualset3
187241	8	415416	7	NULL	NULL	0	NULL	 blood vessels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the effect of CD133 ( + ) cells ( endothelial progenitor cells ) on the hypoxia-induced suppression of axonal growth of cortical neurons and the destruction of blood vessels ( endothelial cells ) , we used anterograde axonal tracing and immunofluorescence in organ co-cultures of the cortex and the spinal cord from 3-day-old neonatal rats .
	manualset3
187242	9	415416	7	NULL	NULL	0	NULL	endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the effect of CD133 ( + ) cells ( endothelial progenitor cells ) on the hypoxia-induced suppression of axonal growth of cortical neurons and the destruction of blood vessels ( endothelial cells ) , we used anterograde axonal tracing and immunofluorescence in organ co-cultures of the cortex and the spinal cord from 3-day-old neonatal rats .
	manualset3
187243	10	415416	7	NULL	NULL	0	NULL	anterograde axonal tracing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the effect of CD133 ( + ) cells ( endothelial progenitor cells ) on the hypoxia-induced suppression of axonal growth of cortical neurons and the destruction of blood vessels ( endothelial cells ) , we used anterograde axonal tracing and immunofluorescence in organ co-cultures of the cortex and the spinal cord from 3-day-old neonatal rats .
	manualset3
187244	11	415416	7	NULL	NULL	0	NULL	immunofluorescence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the effect of CD133 ( + ) cells ( endothelial progenitor cells ) on the hypoxia-induced suppression of axonal growth of cortical neurons and the destruction of blood vessels ( endothelial cells ) , we used anterograde axonal tracing and immunofluorescence in organ co-cultures of the cortex and the spinal cord from 3-day-old neonatal rats .
	manualset3
187245	12	415416	7	NULL	NULL	0	NULL	organ co-cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the effect of CD133 ( + ) cells ( endothelial progenitor cells ) on the hypoxia-induced suppression of axonal growth of cortical neurons and the destruction of blood vessels ( endothelial cells ) , we used anterograde axonal tracing and immunofluorescence in organ co-cultures of the cortex and the spinal cord from 3-day-old neonatal rats .
	manualset3
187246	13	415416	7	NULL	NULL	0	NULL	cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the effect of CD133 ( + ) cells ( endothelial progenitor cells ) on the hypoxia-induced suppression of axonal growth of cortical neurons and the destruction of blood vessels ( endothelial cells ) , we used anterograde axonal tracing and immunofluorescence in organ co-cultures of the cortex and the spinal cord from 3-day-old neonatal rats .
	manualset3
187247	14	415416	7	NULL	NULL	0	NULL	spinal cord	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the effect of CD133 ( + ) cells ( endothelial progenitor cells ) on the hypoxia-induced suppression of axonal growth of cortical neurons and the destruction of blood vessels ( endothelial cells ) , we used anterograde axonal tracing and immunofluorescence in organ co-cultures of the cortex and the spinal cord from 3-day-old neonatal rats .
	manualset3
187248	15	415416	7	NULL	NULL	0	NULL	3-day-old neonatal rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the effect of CD133 ( + ) cells ( endothelial progenitor cells ) on the hypoxia-induced suppression of axonal growth of cortical neurons and the destruction of blood vessels ( endothelial cells ) , we used anterograde axonal tracing and immunofluorescence in organ co-cultures of the cortex and the spinal cord from 3-day-old neonatal rats .
	manualset3
187249	1	415417	7	NULL	NULL	0	NULL	predictive potential	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the predictive potential of the method , we performed 21 drug pair treatment experiments in a human breast cancer cell line ( MCF7 ) with observation of phospho-proteins and cell cycle markers .
	manualset3
187250	2	415417	7	NULL	NULL	0	NULL	method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the predictive potential of the method , we performed 21 drug pair treatment experiments in a human breast cancer cell line ( MCF7 ) with observation of phospho-proteins and cell cycle markers .
	manualset3
187251	3	415417	7	NULL	NULL	NULL	NULL	21 drug pair treatment experiments	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To evaluate the predictive potential of the method , we performed 21 drug pair treatment experiments in a human breast cancer cell line ( MCF7 ) with observation of phospho-proteins and cell cycle markers .
	manualset3
187253	5	415417	7	NULL	NULL	0	NULL	human breast cancer cell line ( MCF7 )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the predictive potential of the method , we performed 21 drug pair treatment experiments in a human breast cancer cell line ( MCF7 ) with observation of phospho-proteins and cell cycle markers .
	manualset3
187254	6	415417	7	NULL	NULL	0	NULL	observation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the predictive potential of the method , we performed 21 drug pair treatment experiments in a human breast cancer cell line ( MCF7 ) with observation of phospho-proteins and cell cycle markers .
	manualset3
187255	7	415417	7	NULL	NULL	NULL	NULL	phospho-proteins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To evaluate the predictive potential of the method , we performed 21 drug pair treatment experiments in a human breast cancer cell line ( MCF7 ) with observation of phospho-proteins and cell cycle markers .
	manualset3
187256	8	415417	7	NULL	NULL	NULL	NULL	cell cycle markers	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To evaluate the predictive potential of the method , we performed 21 drug pair treatment experiments in a human breast cancer cell line ( MCF7 ) with observation of phospho-proteins and cell cycle markers .
	manualset3
187257	1	415418	7	NULL	NULL	0	NULL	relative contributions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the relative contributions of parenchymal cell and bone marrow-derived cell ( BMDC ) B7-H1 expression , we generated and transplanted into WT recipients chimeric liver grafts lacking B7-H1 on parenchymal cells or BMDCs .
	manualset3
187258	2	415418	7	NULL	NULL	0	NULL	parenchymal cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the relative contributions of parenchymal cell and bone marrow-derived cell ( BMDC ) B7-H1 expression , we generated and transplanted into WT recipients chimeric liver grafts lacking B7-H1 on parenchymal cells or BMDCs .
	manualset3
187259	3	415418	7	NULL	NULL	0	NULL	bone marrow-derived cell ( BMDC ) B7-H1 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the relative contributions of parenchymal cell and bone marrow-derived cell ( BMDC ) B7-H1 expression , we generated and transplanted into WT recipients chimeric liver grafts lacking B7-H1 on parenchymal cells or BMDCs .
	manualset3
187260	4	415418	7	NULL	NULL	0	NULL	WT recipients chimeric liver grafts 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the relative contributions of parenchymal cell and bone marrow-derived cell ( BMDC ) B7-H1 expression , we generated and transplanted into WT recipients chimeric liver grafts lacking B7-H1 on parenchymal cells or BMDCs .
	manualset3
187261	5	415418	7	NULL	NULL	0	NULL	B7-H1	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the relative contributions of parenchymal cell and bone marrow-derived cell ( BMDC ) B7-H1 expression , we generated and transplanted into WT recipients chimeric liver grafts lacking B7-H1 on parenchymal cells or BMDCs .
	manualset3
187262	6	415418	7	NULL	NULL	0	NULL	parenchymal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the relative contributions of parenchymal cell and bone marrow-derived cell ( BMDC ) B7-H1 expression , we generated and transplanted into WT recipients chimeric liver grafts lacking B7-H1 on parenchymal cells or BMDCs .
	manualset3
187263	7	415418	7	NULL	NULL	0	NULL	BMDCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the relative contributions of parenchymal cell and bone marrow-derived cell ( BMDC ) B7-H1 expression , we generated and transplanted into WT recipients chimeric liver grafts lacking B7-H1 on parenchymal cells or BMDCs .
	manualset3
187264	1	415419	7	NULL	NULL	0	NULL	cardiac tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine mechanisms by which cardiac tissue regulates the beta-adrenergic receptor and physiological response to beta-adrenergic agonists , we studied the effects of cytoskeletal disrupting agents and inhibition of protein synthesis on receptor properties and contractile response to isoproterenol in intact cultured ventricular cells from embryonic chick heart .
	manualset3
187265	2	415419	7	NULL	NULL	0	NULL	beta-adrenergic receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine mechanisms by which cardiac tissue regulates the beta-adrenergic receptor and physiological response to beta-adrenergic agonists , we studied the effects of cytoskeletal disrupting agents and inhibition of protein synthesis on receptor properties and contractile response to isoproterenol in intact cultured ventricular cells from embryonic chick heart .
	manualset3
187267	3	415419	7	NULL	NULL	0	NULL	physiological response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine mechanisms by which cardiac tissue regulates the beta-adrenergic receptor and physiological response to beta-adrenergic agonists , we studied the effects of cytoskeletal disrupting agents and inhibition of protein synthesis on receptor properties and contractile response to isoproterenol in intact cultured ventricular cells from embryonic chick heart .
	manualset3
187271	4	415419	7	NULL	NULL	0	NULL	beta-adrenergic agonists	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine mechanisms by which cardiac tissue regulates the beta-adrenergic receptor and physiological response to beta-adrenergic agonists , we studied the effects of cytoskeletal disrupting agents and inhibition of protein synthesis on receptor properties and contractile response to isoproterenol in intact cultured ventricular cells from embryonic chick heart .
	manualset3
187275	5	415419	7	NULL	NULL	0	NULL	effects 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine mechanisms by which cardiac tissue regulates the beta-adrenergic receptor and physiological response to beta-adrenergic agonists , we studied the effects of cytoskeletal disrupting agents and inhibition of protein synthesis on receptor properties and contractile response to isoproterenol in intact cultured ventricular cells from embryonic chick heart .
	manualset3
187277	6	415419	7	NULL	NULL	0	NULL	cytoskeletal disrupting agents	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine mechanisms by which cardiac tissue regulates the beta-adrenergic receptor and physiological response to beta-adrenergic agonists , we studied the effects of cytoskeletal disrupting agents and inhibition of protein synthesis on receptor properties and contractile response to isoproterenol in intact cultured ventricular cells from embryonic chick heart .
	manualset3
187280	7	415419	7	NULL	NULL	0	NULL	inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine mechanisms by which cardiac tissue regulates the beta-adrenergic receptor and physiological response to beta-adrenergic agonists , we studied the effects of cytoskeletal disrupting agents and inhibition of protein synthesis on receptor properties and contractile response to isoproterenol in intact cultured ventricular cells from embryonic chick heart .
	manualset3
187282	8	415419	7	NULL	NULL	0	NULL	protein synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine mechanisms by which cardiac tissue regulates the beta-adrenergic receptor and physiological response to beta-adrenergic agonists , we studied the effects of cytoskeletal disrupting agents and inhibition of protein synthesis on receptor properties and contractile response to isoproterenol in intact cultured ventricular cells from embryonic chick heart .
	manualset3
187284	9	415419	7	NULL	NULL	0	NULL	 receptor properties 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine mechanisms by which cardiac tissue regulates the beta-adrenergic receptor and physiological response to beta-adrenergic agonists , we studied the effects of cytoskeletal disrupting agents and inhibition of protein synthesis on receptor properties and contractile response to isoproterenol in intact cultured ventricular cells from embryonic chick heart .
	manualset3
187286	10	415419	7	NULL	NULL	0	NULL	 contractile response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine mechanisms by which cardiac tissue regulates the beta-adrenergic receptor and physiological response to beta-adrenergic agonists , we studied the effects of cytoskeletal disrupting agents and inhibition of protein synthesis on receptor properties and contractile response to isoproterenol in intact cultured ventricular cells from embryonic chick heart .
	manualset3
187289	11	415419	7	NULL	NULL	0	NULL	isoproterenol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine mechanisms by which cardiac tissue regulates the beta-adrenergic receptor and physiological response to beta-adrenergic agonists , we studied the effects of cytoskeletal disrupting agents and inhibition of protein synthesis on receptor properties and contractile response to isoproterenol in intact cultured ventricular cells from embryonic chick heart .
	manualset3
187290	12	415419	7	NULL	NULL	0	NULL	intact cultured ventricular cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine mechanisms by which cardiac tissue regulates the beta-adrenergic receptor and physiological response to beta-adrenergic agonists , we studied the effects of cytoskeletal disrupting agents and inhibition of protein synthesis on receptor properties and contractile response to isoproterenol in intact cultured ventricular cells from embryonic chick heart .
	manualset3
187292	13	415419	7	NULL	NULL	0	NULL	embryonic chick heart	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine mechanisms by which cardiac tissue regulates the beta-adrenergic receptor and physiological response to beta-adrenergic agonists , we studied the effects of cytoskeletal disrupting agents and inhibition of protein synthesis on receptor properties and contractile response to isoproterenol in intact cultured ventricular cells from embryonic chick heart .
	manualset3
187295	14	415419	7	NULL	NULL	0	NULL	mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine mechanisms by which cardiac tissue regulates the beta-adrenergic receptor and physiological response to beta-adrenergic agonists , we studied the effects of cytoskeletal disrupting agents and inhibition of protein synthesis on receptor properties and contractile response to isoproterenol in intact cultured ventricular cells from embryonic chick heart .
	manualset3
187299	1	415420	7	NULL	NULL	0	NULL	effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine the effects of growth hormone ( GH ) on the preferential atrophy of the soleus muscle ( SOL ) occurring after hindlimb suspension ( HS ) , two groups of male rats received daily injections of 2 IU.kg-1 body mass of recombinant human growth hormone ( rhGH ) .
	manualset3
187301	2	415420	7	NULL	NULL	0	NULL	growth hormone ( GH )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine the effects of growth hormone ( GH ) on the preferential atrophy of the soleus muscle ( SOL ) occurring after hindlimb suspension ( HS ) , two groups of male rats received daily injections of 2 IU.kg-1 body mass of recombinant human growth hormone ( rhGH ) .
	manualset3
187303	3	415420	7	NULL	NULL	0	NULL	preferential atrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine the effects of growth hormone ( GH ) on the preferential atrophy of the soleus muscle ( SOL ) occurring after hindlimb suspension ( HS ) , two groups of male rats received daily injections of 2 IU.kg-1 body mass of recombinant human growth hormone ( rhGH ) .
	manualset3
187304	4	415420	7	NULL	NULL	0	NULL	soleus muscle ( SOL ) 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine the effects of growth hormone ( GH ) on the preferential atrophy of the soleus muscle ( SOL ) occurring after hindlimb suspension ( HS ) , two groups of male rats received daily injections of 2 IU.kg-1 body mass of recombinant human growth hormone ( rhGH ) .
	manualset3
187305	5	415420	7	NULL	NULL	0	NULL	hindlimb suspension ( HS )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine the effects of growth hormone ( GH ) on the preferential atrophy of the soleus muscle ( SOL ) occurring after hindlimb suspension ( HS ) , two groups of male rats received daily injections of 2 IU.kg-1 body mass of recombinant human growth hormone ( rhGH ) .
	manualset3
187306	6	415420	7	NULL	NULL	0	NULL	two groups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine the effects of growth hormone ( GH ) on the preferential atrophy of the soleus muscle ( SOL ) occurring after hindlimb suspension ( HS ) , two groups of male rats received daily injections of 2 IU.kg-1 body mass of recombinant human growth hormone ( rhGH ) .
	manualset3
187307	7	415420	7	NULL	NULL	0	NULL	male rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine the effects of growth hormone ( GH ) on the preferential atrophy of the soleus muscle ( SOL ) occurring after hindlimb suspension ( HS ) , two groups of male rats received daily injections of 2 IU.kg-1 body mass of recombinant human growth hormone ( rhGH ) .
	manualset3
187308	8	415420	7	NULL	NULL	0	NULL	daily injections 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine the effects of growth hormone ( GH ) on the preferential atrophy of the soleus muscle ( SOL ) occurring after hindlimb suspension ( HS ) , two groups of male rats received daily injections of 2 IU.kg-1 body mass of recombinant human growth hormone ( rhGH ) .
	manualset3
187310	9	415420	7	NULL	NULL	0	NULL	2 IU.kg-1 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine the effects of growth hormone ( GH ) on the preferential atrophy of the soleus muscle ( SOL ) occurring after hindlimb suspension ( HS ) , two groups of male rats received daily injections of 2 IU.kg-1 body mass of recombinant human growth hormone ( rhGH ) .
	manualset3
187312	10	415420	7	NULL	NULL	0	NULL	body mass	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine the effects of growth hormone ( GH ) on the preferential atrophy of the soleus muscle ( SOL ) occurring after hindlimb suspension ( HS ) , two groups of male rats received daily injections of 2 IU.kg-1 body mass of recombinant human growth hormone ( rhGH ) .
	manualset3
187313	11	415420	7	NULL	NULL	0	NULL	recombinant human growth hormone ( rhGH )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine the effects of growth hormone ( GH ) on the preferential atrophy of the soleus muscle ( SOL ) occurring after hindlimb suspension ( HS ) , two groups of male rats received daily injections of 2 IU.kg-1 body mass of recombinant human growth hormone ( rhGH ) .
	manualset3
187315	1	415421	7	NULL	NULL	0	NULL	seven decades	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After almost seven decades in clinical use , aminoglycoside antibiotics still remain indispensible drugs for acute infections and specific indications such as tuberculosis or the containment of pseudomonas bacteria in patients with cystic fibrosis .
	manualset3
187316	2	415421	7	NULL	NULL	0	NULL	aminoglycoside antibiotics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	After almost seven decades in clinical use , aminoglycoside antibiotics still remain indispensible drugs for acute infections and specific indications such as tuberculosis or the containment of pseudomonas bacteria in patients with cystic fibrosis .
	manualset3
187317	3	415421	7	NULL	NULL	0	NULL	indispensible drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	After almost seven decades in clinical use , aminoglycoside antibiotics still remain indispensible drugs for acute infections and specific indications such as tuberculosis or the containment of pseudomonas bacteria in patients with cystic fibrosis .
	manualset3
187318	4	415421	7	NULL	NULL	0	NULL	acute infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After almost seven decades in clinical use , aminoglycoside antibiotics still remain indispensible drugs for acute infections and specific indications such as tuberculosis or the containment of pseudomonas bacteria in patients with cystic fibrosis .
	manualset3
187319	5	415421	7	NULL	NULL	0	NULL	specific indications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After almost seven decades in clinical use , aminoglycoside antibiotics still remain indispensible drugs for acute infections and specific indications such as tuberculosis or the containment of pseudomonas bacteria in patients with cystic fibrosis .
	manualset3
187321	6	415421	7	NULL	NULL	0	NULL	tuberculosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	After almost seven decades in clinical use , aminoglycoside antibiotics still remain indispensible drugs for acute infections and specific indications such as tuberculosis or the containment of pseudomonas bacteria in patients with cystic fibrosis .
	manualset3
187322	7	415421	7	NULL	NULL	0	NULL	containment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After almost seven decades in clinical use , aminoglycoside antibiotics still remain indispensible drugs for acute infections and specific indications such as tuberculosis or the containment of pseudomonas bacteria in patients with cystic fibrosis .
	manualset3
187324	8	415421	7	NULL	NULL	0	NULL	pseudomonas bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	After almost seven decades in clinical use , aminoglycoside antibiotics still remain indispensible drugs for acute infections and specific indications such as tuberculosis or the containment of pseudomonas bacteria in patients with cystic fibrosis .
	manualset3
187326	9	415421	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	After almost seven decades in clinical use , aminoglycoside antibiotics still remain indispensible drugs for acute infections and specific indications such as tuberculosis or the containment of pseudomonas bacteria in patients with cystic fibrosis .
	manualset3
187327	10	415421	7	NULL	NULL	0	NULL	cystic fibrosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	After almost seven decades in clinical use , aminoglycoside antibiotics still remain indispensible drugs for acute infections and specific indications such as tuberculosis or the containment of pseudomonas bacteria in patients with cystic fibrosis .
	manualset3
187328	1	415422	7	NULL	NULL	0	NULL	relevance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine the relevance of these data to the in vivo state , rats were injected with ( 32P ) orthophosphate .
	manualset3
187330	2	415422	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine the relevance of these data to the in vivo state , rats were injected with ( 32P ) orthophosphate .
	manualset3
187332	3	415422	7	NULL	NULL	0	NULL	in vivo state	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine the relevance of these data to the in vivo state , rats were injected with ( 32P ) orthophosphate .
	manualset3
187334	4	415422	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine the relevance of these data to the in vivo state , rats were injected with ( 32P ) orthophosphate .
	manualset3
187336	5	415422	7	NULL	NULL	0	NULL	( 32P ) orthophosphate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine the relevance of these data to the in vivo state , rats were injected with ( 32P ) orthophosphate .
	manualset3
187354	1	415423	7	NULL	NULL	0	NULL	 unfolding reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine this unfolding reaction , we have prepared proOmpA-Dhfr , a fusion protein of the well studied cytosolic enzyme dihydrofolate reductase ( Dhfr ) connected to the C-terminus of proOmpA , the precursor form of outer membrane protein A. At an intermediate stage of its in vitro translocation , the N-terminal proOmpA domain has crossed the membrane while the folded Dhfr portion , stabilized by its ligands NADPH and methotrexate , has not .
	manualset3
187355	2	415423	7	NULL	NULL	0	NULL	proOmpA-Dhfr	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine this unfolding reaction , we have prepared proOmpA-Dhfr , a fusion protein of the well studied cytosolic enzyme dihydrofolate reductase ( Dhfr ) connected to the C-terminus of proOmpA , the precursor form of outer membrane protein A. At an intermediate stage of its in vitro translocation , the N-terminal proOmpA domain has crossed the membrane while the folded Dhfr portion , stabilized by its ligands NADPH and methotrexate , has not .
	manualset3
187356	3	415423	7	NULL	NULL	0	NULL	fusion protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine this unfolding reaction , we have prepared proOmpA-Dhfr , a fusion protein of the well studied cytosolic enzyme dihydrofolate reductase ( Dhfr ) connected to the C-terminus of proOmpA , the precursor form of outer membrane protein A. At an intermediate stage of its in vitro translocation , the N-terminal proOmpA domain has crossed the membrane while the folded Dhfr portion , stabilized by its ligands NADPH and methotrexate , has not .
	manualset3
187357	4	415423	7	NULL	NULL	0	NULL	cytosolic enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine this unfolding reaction , we have prepared proOmpA-Dhfr , a fusion protein of the well studied cytosolic enzyme dihydrofolate reductase ( Dhfr ) connected to the C-terminus of proOmpA , the precursor form of outer membrane protein A. At an intermediate stage of its in vitro translocation , the N-terminal proOmpA domain has crossed the membrane while the folded Dhfr portion , stabilized by its ligands NADPH and methotrexate , has not .
	manualset3
187358	5	415423	7	NULL	NULL	0	NULL	dihydrofolate reductase ( Dhfr )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine this unfolding reaction , we have prepared proOmpA-Dhfr , a fusion protein of the well studied cytosolic enzyme dihydrofolate reductase ( Dhfr ) connected to the C-terminus of proOmpA , the precursor form of outer membrane protein A. At an intermediate stage of its in vitro translocation , the N-terminal proOmpA domain has crossed the membrane while the folded Dhfr portion , stabilized by its ligands NADPH and methotrexate , has not .
	manualset3
187359	6	415423	7	NULL	NULL	0	NULL	C-terminus	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine this unfolding reaction , we have prepared proOmpA-Dhfr , a fusion protein of the well studied cytosolic enzyme dihydrofolate reductase ( Dhfr ) connected to the C-terminus of proOmpA , the precursor form of outer membrane protein A. At an intermediate stage of its in vitro translocation , the N-terminal proOmpA domain has crossed the membrane while the folded Dhfr portion , stabilized by its ligands NADPH and methotrexate , has not .
	manualset3
187360	7	415423	7	NULL	NULL	0	NULL	proOmpA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine this unfolding reaction , we have prepared proOmpA-Dhfr , a fusion protein of the well studied cytosolic enzyme dihydrofolate reductase ( Dhfr ) connected to the C-terminus of proOmpA , the precursor form of outer membrane protein A. At an intermediate stage of its in vitro translocation , the N-terminal proOmpA domain has crossed the membrane while the folded Dhfr portion , stabilized by its ligands NADPH and methotrexate , has not .
	manualset3
187361	8	415423	7	NULL	NULL	0	NULL	precursor form	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine this unfolding reaction , we have prepared proOmpA-Dhfr , a fusion protein of the well studied cytosolic enzyme dihydrofolate reductase ( Dhfr ) connected to the C-terminus of proOmpA , the precursor form of outer membrane protein A. At an intermediate stage of its in vitro translocation , the N-terminal proOmpA domain has crossed the membrane while the folded Dhfr portion , stabilized by its ligands NADPH and methotrexate , has not .
	manualset3
187362	9	415423	7	NULL	NULL	0	NULL	outer membrane protein A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine this unfolding reaction , we have prepared proOmpA-Dhfr , a fusion protein of the well studied cytosolic enzyme dihydrofolate reductase ( Dhfr ) connected to the C-terminus of proOmpA , the precursor form of outer membrane protein A. At an intermediate stage of its in vitro translocation , the N-terminal proOmpA domain has crossed the membrane while the folded Dhfr portion , stabilized by its ligands NADPH and methotrexate , has not .
	manualset3
187363	10	415423	7	NULL	NULL	0	NULL	 intermediate stage 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine this unfolding reaction , we have prepared proOmpA-Dhfr , a fusion protein of the well studied cytosolic enzyme dihydrofolate reductase ( Dhfr ) connected to the C-terminus of proOmpA , the precursor form of outer membrane protein A. At an intermediate stage of its in vitro translocation , the N-terminal proOmpA domain has crossed the membrane while the folded Dhfr portion , stabilized by its ligands NADPH and methotrexate , has not .
	manualset3
187364	11	415423	7	NULL	NULL	0	NULL	in vitro translocation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine this unfolding reaction , we have prepared proOmpA-Dhfr , a fusion protein of the well studied cytosolic enzyme dihydrofolate reductase ( Dhfr ) connected to the C-terminus of proOmpA , the precursor form of outer membrane protein A. At an intermediate stage of its in vitro translocation , the N-terminal proOmpA domain has crossed the membrane while the folded Dhfr portion , stabilized by its ligands NADPH and methotrexate , has not .
	manualset3
187365	12	415423	7	NULL	NULL	0	NULL	N-terminal proOmpA domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine this unfolding reaction , we have prepared proOmpA-Dhfr , a fusion protein of the well studied cytosolic enzyme dihydrofolate reductase ( Dhfr ) connected to the C-terminus of proOmpA , the precursor form of outer membrane protein A. At an intermediate stage of its in vitro translocation , the N-terminal proOmpA domain has crossed the membrane while the folded Dhfr portion , stabilized by its ligands NADPH and methotrexate , has not .
	manualset3
187366	13	415423	7	NULL	NULL	0	NULL	membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine this unfolding reaction , we have prepared proOmpA-Dhfr , a fusion protein of the well studied cytosolic enzyme dihydrofolate reductase ( Dhfr ) connected to the C-terminus of proOmpA , the precursor form of outer membrane protein A. At an intermediate stage of its in vitro translocation , the N-terminal proOmpA domain has crossed the membrane while the folded Dhfr portion , stabilized by its ligands NADPH and methotrexate , has not .
	manualset3
187367	14	415423	7	NULL	NULL	0	NULL	folded Dhfr portion	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine this unfolding reaction , we have prepared proOmpA-Dhfr , a fusion protein of the well studied cytosolic enzyme dihydrofolate reductase ( Dhfr ) connected to the C-terminus of proOmpA , the precursor form of outer membrane protein A. At an intermediate stage of its in vitro translocation , the N-terminal proOmpA domain has crossed the membrane while the folded Dhfr portion , stabilized by its ligands NADPH and methotrexate , has not .
	manualset3
187368	15	415423	7	NULL	NULL	0	NULL	ligands NADPH	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine this unfolding reaction , we have prepared proOmpA-Dhfr , a fusion protein of the well studied cytosolic enzyme dihydrofolate reductase ( Dhfr ) connected to the C-terminus of proOmpA , the precursor form of outer membrane protein A. At an intermediate stage of its in vitro translocation , the N-terminal proOmpA domain has crossed the membrane while the folded Dhfr portion , stabilized by its ligands NADPH and methotrexate , has not .
	manualset3
187369	16	415423	7	NULL	NULL	0	NULL	methotrexate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine this unfolding reaction , we have prepared proOmpA-Dhfr , a fusion protein of the well studied cytosolic enzyme dihydrofolate reductase ( Dhfr ) connected to the C-terminus of proOmpA , the precursor form of outer membrane protein A. At an intermediate stage of its in vitro translocation , the N-terminal proOmpA domain has crossed the membrane while the folded Dhfr portion , stabilized by its ligands NADPH and methotrexate , has not .
	manualset3
187370	1	415424	7	NULL	NULL	NULL	NULL	types of sequences	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To examine what types of sequences from mouse genomic DNA bind to EVI1 , we isolated and sequenced five EVI1-binding fragments , and each showed the GACAAGATA site .
	manualset3
187371	2	415424	7	NULL	NULL	0	NULL	mouse genomic DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine what types of sequences from mouse genomic DNA bind to EVI1 , we isolated and sequenced five EVI1-binding fragments , and each showed the GACAAGATA site .
	manualset3
187372	3	415424	7	NULL	NULL	0	NULL	EVI1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine what types of sequences from mouse genomic DNA bind to EVI1 , we isolated and sequenced five EVI1-binding fragments , and each showed the GACAAGATA site .
	manualset3
187373	4	415424	7	NULL	NULL	0	NULL	 five	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine what types of sequences from mouse genomic DNA bind to EVI1 , we isolated and sequenced five EVI1-binding fragments , and each showed the GACAAGATA site .
	manualset3
187374	5	415424	7	NULL	NULL	0	NULL	EVI1-binding fragments	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine what types of sequences from mouse genomic DNA bind to EVI1 , we isolated and sequenced five EVI1-binding fragments , and each showed the GACAAGATA site .
	manualset3
187375	6	415424	7	NULL	NULL	0	NULL	GACAAGATA site	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine what types of sequences from mouse genomic DNA bind to EVI1 , we isolated and sequenced five EVI1-binding fragments , and each showed the GACAAGATA site .
	manualset3
187376	1	415425	7	NULL	NULL	0	NULL	new treatment strategy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore a new treatment strategy for urinary incontinence , human bone marrow mesenchymal stem cells ( MSC ) of the first in vitro passage were exposed to 5-azacytidine ( AZA ) to induce myogenic differentiation , and cultured for a total of six passages .
	manualset3
187377	2	415425	7	NULL	NULL	0	NULL	urinary incontinence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore a new treatment strategy for urinary incontinence , human bone marrow mesenchymal stem cells ( MSC ) of the first in vitro passage were exposed to 5-azacytidine ( AZA ) to induce myogenic differentiation , and cultured for a total of six passages .
	manualset3
187378	3	415425	7	NULL	NULL	0	NULL	human bone marrow mesenchymal stem cells ( MSC )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore a new treatment strategy for urinary incontinence , human bone marrow mesenchymal stem cells ( MSC ) of the first in vitro passage were exposed to 5-azacytidine ( AZA ) to induce myogenic differentiation , and cultured for a total of six passages .
	manualset3
187379	4	415425	7	NULL	NULL	0	NULL	in vitro passage	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore a new treatment strategy for urinary incontinence , human bone marrow mesenchymal stem cells ( MSC ) of the first in vitro passage were exposed to 5-azacytidine ( AZA ) to induce myogenic differentiation , and cultured for a total of six passages .
	manualset3
187380	5	415425	7	NULL	NULL	0	NULL	5-azacytidine ( AZA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore a new treatment strategy for urinary incontinence , human bone marrow mesenchymal stem cells ( MSC ) of the first in vitro passage were exposed to 5-azacytidine ( AZA ) to induce myogenic differentiation , and cultured for a total of six passages .
	manualset3
187381	6	415425	7	NULL	NULL	0	NULL	myogenic differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore a new treatment strategy for urinary incontinence , human bone marrow mesenchymal stem cells ( MSC ) of the first in vitro passage were exposed to 5-azacytidine ( AZA ) to induce myogenic differentiation , and cultured for a total of six passages .
	manualset3
187382	7	415425	7	NULL	NULL	0	NULL	total 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore a new treatment strategy for urinary incontinence , human bone marrow mesenchymal stem cells ( MSC ) of the first in vitro passage were exposed to 5-azacytidine ( AZA ) to induce myogenic differentiation , and cultured for a total of six passages .
	manualset3
187383	8	415425	7	NULL	NULL	0	NULL	six passages 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore a new treatment strategy for urinary incontinence , human bone marrow mesenchymal stem cells ( MSC ) of the first in vitro passage were exposed to 5-azacytidine ( AZA ) to induce myogenic differentiation , and cultured for a total of six passages .
	manualset3
187384	1	415426	7	NULL	NULL	0	NULL	interspecies interactions 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore such interspecies interactions , we focused on Bacillus subtilis , which characteristically develops into matrix-producing cannibals before entering sporulation .
	manualset3
187385	2	415426	7	NULL	NULL	0	NULL	Bacillus subtilis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore such interspecies interactions , we focused on Bacillus subtilis , which characteristically develops into matrix-producing cannibals before entering sporulation .
	manualset3
187386	3	415426	7	NULL	NULL	0	NULL	matrix-producing cannibals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore such interspecies interactions , we focused on Bacillus subtilis , which characteristically develops into matrix-producing cannibals before entering sporulation .
	manualset3
187387	4	415426	7	NULL	NULL	0	NULL	sporulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore such interspecies interactions , we focused on Bacillus subtilis , which characteristically develops into matrix-producing cannibals before entering sporulation .
	manualset3
187388	1	415427	7	NULL	NULL	0	NULL	 influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the influence of the deformity on occlusion , the skulls were categorized using the Angle classification and the alignment of the interincisor midline .
	manualset3
187389	2	415427	7	NULL	NULL	0	NULL	deformity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the influence of the deformity on occlusion , the skulls were categorized using the Angle classification and the alignment of the interincisor midline .
	manualset3
187390	3	415427	7	NULL	NULL	0	NULL	 occlusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the influence of the deformity on occlusion , the skulls were categorized using the Angle classification and the alignment of the interincisor midline .
	manualset3
187391	4	415427	7	NULL	NULL	0	NULL	skulls 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the influence of the deformity on occlusion , the skulls were categorized using the Angle classification and the alignment of the interincisor midline .
	manualset3
187392	5	415427	7	NULL	NULL	0	NULL	Angle classification	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the influence of the deformity on occlusion , the skulls were categorized using the Angle classification and the alignment of the interincisor midline .
	manualset3
187393	6	415427	7	NULL	NULL	0	NULL	alignment	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the influence of the deformity on occlusion , the skulls were categorized using the Angle classification and the alignment of the interincisor midline .
	manualset3
187394	7	415427	7	NULL	NULL	0	NULL	interincisor midline	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the influence of the deformity on occlusion , the skulls were categorized using the Angle classification and the alignment of the interincisor midline .
	manualset3
187395	1	415428	7	NULL	NULL	0	NULL	mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the mechanism of constitutive IL-2 expression in MLA 144 , we have isolated and characterized cosmid clones representing a normal and a doubly inserted IL-2 allele in this cell line .
	manualset3
187396	2	415428	7	NULL	NULL	0	NULL	constitutive IL-2 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the mechanism of constitutive IL-2 expression in MLA 144 , we have isolated and characterized cosmid clones representing a normal and a doubly inserted IL-2 allele in this cell line .
	manualset3
187397	3	415428	7	NULL	NULL	0	NULL	MLA 144	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the mechanism of constitutive IL-2 expression in MLA 144 , we have isolated and characterized cosmid clones representing a normal and a doubly inserted IL-2 allele in this cell line .
	manualset3
187398	4	415428	7	NULL	NULL	0	NULL	cosmid clones	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the mechanism of constitutive IL-2 expression in MLA 144 , we have isolated and characterized cosmid clones representing a normal and a doubly inserted IL-2 allele in this cell line .
	manualset3
187399	5	415428	7	NULL	NULL	0	NULL	normal allele	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the mechanism of constitutive IL-2 expression in MLA 144 , we have isolated and characterized cosmid clones representing a normal and a doubly inserted IL-2 allele in this cell line .
	manualset3
187400	6	415428	7	NULL	NULL	0	NULL	doubly inserted IL-2 allele	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the mechanism of constitutive IL-2 expression in MLA 144 , we have isolated and characterized cosmid clones representing a normal and a doubly inserted IL-2 allele in this cell line .
	manualset3
187401	7	415428	7	NULL	NULL	0	NULL	cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the mechanism of constitutive IL-2 expression in MLA 144 , we have isolated and characterized cosmid clones representing a normal and a doubly inserted IL-2 allele in this cell line .
	manualset3
187404	1	415429	7	NULL	NULL	0	NULL	problem	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the problem of type I ( false-positive ) statistical errors associated with enumerating endocrine pulses , we used the analysis of immunoactive luteinizing hormone ( LH ) pulses as a paradigm .
	manualset3
187406	2	415429	7	NULL	NULL	0	NULL	type I ( false-positive ) statistical errors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the problem of type I ( false-positive ) statistical errors associated with enumerating endocrine pulses , we used the analysis of immunoactive luteinizing hormone ( LH ) pulses as a paradigm .
	manualset3
187408	3	415429	7	NULL	NULL	0	NULL	endocrine pulses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the problem of type I ( false-positive ) statistical errors associated with enumerating endocrine pulses , we used the analysis of immunoactive luteinizing hormone ( LH ) pulses as a paradigm .
	manualset3
187409	4	415429	7	NULL	NULL	0	NULL	 analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the problem of type I ( false-positive ) statistical errors associated with enumerating endocrine pulses , we used the analysis of immunoactive luteinizing hormone ( LH ) pulses as a paradigm .
	manualset3
187411	5	415429	7	NULL	NULL	0	NULL	immunoactive luteinizing hormone ( LH ) pulses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the problem of type I ( false-positive ) statistical errors associated with enumerating endocrine pulses , we used the analysis of immunoactive luteinizing hormone ( LH ) pulses as a paradigm .
	manualset3
187413	1	415430	7	NULL	NULL	0	NULL	 role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the role of Akt1 in mammary gland function and tumorigenesis , transgenic mice were generated that express human AKT1 under the control of the MMTV promoter .
	manualset3
187414	2	415430	7	NULL	NULL	0	NULL	Akt1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the role of Akt1 in mammary gland function and tumorigenesis , transgenic mice were generated that express human AKT1 under the control of the MMTV promoter .
	manualset3
187415	3	415430	7	NULL	NULL	0	NULL	mammary gland function 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the role of Akt1 in mammary gland function and tumorigenesis , transgenic mice were generated that express human AKT1 under the control of the MMTV promoter .
	manualset3
187416	4	415430	7	NULL	NULL	0	NULL	tumorigenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the role of Akt1 in mammary gland function and tumorigenesis , transgenic mice were generated that express human AKT1 under the control of the MMTV promoter .
	manualset3
187417	5	415430	7	NULL	NULL	0	NULL	transgenic mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the role of Akt1 in mammary gland function and tumorigenesis , transgenic mice were generated that express human AKT1 under the control of the MMTV promoter .
	manualset3
187418	6	415430	7	NULL	NULL	0	NULL	human AKT1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the role of Akt1 in mammary gland function and tumorigenesis , transgenic mice were generated that express human AKT1 under the control of the MMTV promoter .
	manualset3
187420	7	415430	7	NULL	NULL	0	NULL	control 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the role of Akt1 in mammary gland function and tumorigenesis , transgenic mice were generated that express human AKT1 under the control of the MMTV promoter .
	manualset3
187421	8	415430	7	NULL	NULL	0	NULL	MMTV promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the role of Akt1 in mammary gland function and tumorigenesis , transgenic mice were generated that express human AKT1 under the control of the MMTV promoter .
	manualset3
187592	1	415431	7	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the role of Pgp in drug transport across an endothelial cell barrier derived from the central nervous system , the expression and activity of Pgp in bovine retinal endothelial cells ( BRECs ) and the effects of representative CNS drugs on Pgp activity were examined .
	manualset3
187593	2	415431	7	NULL	NULL	0	NULL	Pgp	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the role of Pgp in drug transport across an endothelial cell barrier derived from the central nervous system , the expression and activity of Pgp in bovine retinal endothelial cells ( BRECs ) and the effects of representative CNS drugs on Pgp activity were examined .
	manualset3
187595	3	415431	7	NULL	NULL	0	NULL	drug transport 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the role of Pgp in drug transport across an endothelial cell barrier derived from the central nervous system , the expression and activity of Pgp in bovine retinal endothelial cells ( BRECs ) and the effects of representative CNS drugs on Pgp activity were examined .
	manualset3
187597	4	415431	7	NULL	NULL	0	NULL	endothelial cell barrier	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the role of Pgp in drug transport across an endothelial cell barrier derived from the central nervous system , the expression and activity of Pgp in bovine retinal endothelial cells ( BRECs ) and the effects of representative CNS drugs on Pgp activity were examined .
	manualset3
187598	5	415431	7	NULL	NULL	0	NULL	central nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the role of Pgp in drug transport across an endothelial cell barrier derived from the central nervous system , the expression and activity of Pgp in bovine retinal endothelial cells ( BRECs ) and the effects of representative CNS drugs on Pgp activity were examined .
	manualset3
187601	6	415431	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the role of Pgp in drug transport across an endothelial cell barrier derived from the central nervous system , the expression and activity of Pgp in bovine retinal endothelial cells ( BRECs ) and the effects of representative CNS drugs on Pgp activity were examined .
	manualset3
187603	7	415431	7	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the role of Pgp in drug transport across an endothelial cell barrier derived from the central nervous system , the expression and activity of Pgp in bovine retinal endothelial cells ( BRECs ) and the effects of representative CNS drugs on Pgp activity were examined .
	manualset3
187605	8	415431	7	NULL	NULL	0	NULL	Pgp	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the role of Pgp in drug transport across an endothelial cell barrier derived from the central nervous system , the expression and activity of Pgp in bovine retinal endothelial cells ( BRECs ) and the effects of representative CNS drugs on Pgp activity were examined .
	manualset3
187607	9	415431	7	NULL	NULL	0	NULL	bovine retinal endothelial cells ( BRECs )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the role of Pgp in drug transport across an endothelial cell barrier derived from the central nervous system , the expression and activity of Pgp in bovine retinal endothelial cells ( BRECs ) and the effects of representative CNS drugs on Pgp activity were examined .
	manualset3
187608	10	415431	7	NULL	NULL	0	NULL	effects 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the role of Pgp in drug transport across an endothelial cell barrier derived from the central nervous system , the expression and activity of Pgp in bovine retinal endothelial cells ( BRECs ) and the effects of representative CNS drugs on Pgp activity were examined .
	manualset3
187609	11	415431	7	NULL	NULL	0	NULL	CNS drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the role of Pgp in drug transport across an endothelial cell barrier derived from the central nervous system , the expression and activity of Pgp in bovine retinal endothelial cells ( BRECs ) and the effects of representative CNS drugs on Pgp activity were examined .
	manualset3
187611	12	415431	7	NULL	NULL	0	NULL	Pgp activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To explore the role of Pgp in drug transport across an endothelial cell barrier derived from the central nervous system , the expression and activity of Pgp in bovine retinal endothelial cells ( BRECs ) and the effects of representative CNS drugs on Pgp activity were examined .
	manualset3
187615	1	415432	7	NULL	NULL	0	NULL	understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To extend our current understanding of the underlying limitations of such approaches , we performed quantitative uptake studies of different chemically modified ( 2 ' - O-methyl , LNA and PNA ) steric block oligonucleotides , targeted against a mutated splice site inserted in a firefly luciferase reporter gene construct , applying the peptide carrier MPGalpha as a model system .
	manualset3
187619	2	415432	7	NULL	NULL	0	NULL	underlying limitations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To extend our current understanding of the underlying limitations of such approaches , we performed quantitative uptake studies of different chemically modified ( 2 ' - O-methyl , LNA and PNA ) steric block oligonucleotides , targeted against a mutated splice site inserted in a firefly luciferase reporter gene construct , applying the peptide carrier MPGalpha as a model system .
	manualset3
187620	3	415432	7	NULL	NULL	0	NULL	approaches	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To extend our current understanding of the underlying limitations of such approaches , we performed quantitative uptake studies of different chemically modified ( 2 ' - O-methyl , LNA and PNA ) steric block oligonucleotides , targeted against a mutated splice site inserted in a firefly luciferase reporter gene construct , applying the peptide carrier MPGalpha as a model system .
	manualset3
187621	4	415432	7	NULL	NULL	0	NULL	quantitative uptake studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To extend our current understanding of the underlying limitations of such approaches , we performed quantitative uptake studies of different chemically modified ( 2 ' - O-methyl , LNA and PNA ) steric block oligonucleotides , targeted against a mutated splice site inserted in a firefly luciferase reporter gene construct , applying the peptide carrier MPGalpha as a model system .
	manualset3
187622	5	415432	7	NULL	NULL	0	NULL	chemically modified ( 2 ' - O-methyl , LNA and PNA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To extend our current understanding of the underlying limitations of such approaches , we performed quantitative uptake studies of different chemically modified ( 2 ' - O-methyl , LNA and PNA ) steric block oligonucleotides , targeted against a mutated splice site inserted in a firefly luciferase reporter gene construct , applying the peptide carrier MPGalpha as a model system .
	manualset3
187623	6	415432	7	NULL	NULL	0	NULL	steric block oligonucleotides	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To extend our current understanding of the underlying limitations of such approaches , we performed quantitative uptake studies of different chemically modified ( 2 ' - O-methyl , LNA and PNA ) steric block oligonucleotides , targeted against a mutated splice site inserted in a firefly luciferase reporter gene construct , applying the peptide carrier MPGalpha as a model system .
	manualset3
187624	7	415432	7	NULL	NULL	0	NULL	mutated splice site	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To extend our current understanding of the underlying limitations of such approaches , we performed quantitative uptake studies of different chemically modified ( 2 ' - O-methyl , LNA and PNA ) steric block oligonucleotides , targeted against a mutated splice site inserted in a firefly luciferase reporter gene construct , applying the peptide carrier MPGalpha as a model system .
	manualset3
187625	8	415432	7	NULL	NULL	0	NULL	firefly luciferase reporter gene construct	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	To extend our current understanding of the underlying limitations of such approaches , we performed quantitative uptake studies of different chemically modified ( 2 ' - O-methyl , LNA and PNA ) steric block oligonucleotides , targeted against a mutated splice site inserted in a firefly luciferase reporter gene construct , applying the peptide carrier MPGalpha as a model system .
	manualset3
187626	9	415432	7	NULL	NULL	0	NULL	peptide carrier MPGalpha	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To extend our current understanding of the underlying limitations of such approaches , we performed quantitative uptake studies of different chemically modified ( 2 ' - O-methyl , LNA and PNA ) steric block oligonucleotides , targeted against a mutated splice site inserted in a firefly luciferase reporter gene construct , applying the peptide carrier MPGalpha as a model system .
	manualset3
187627	10	415432	7	NULL	NULL	0	NULL	model system 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To extend our current understanding of the underlying limitations of such approaches , we performed quantitative uptake studies of different chemically modified ( 2 ' - O-methyl , LNA and PNA ) steric block oligonucleotides , targeted against a mutated splice site inserted in a firefly luciferase reporter gene construct , applying the peptide carrier MPGalpha as a model system .
	manualset3
188221	1	415433	7	NULL	NULL	0	NULL	networked discovery	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To facilitate networked discovery and information retrieval in the biomedical domain , we have designed a system for automatic assignment of Medical Subject Headings to documents retrieved from the World-Wide Web .
	manualset3
188222	2	415433	7	NULL	NULL	0	NULL	information retrieval	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To facilitate networked discovery and information retrieval in the biomedical domain , we have designed a system for automatic assignment of Medical Subject Headings to documents retrieved from the World-Wide Web .
	manualset3
188223	3	415433	7	NULL	NULL	0	NULL	biomedical domain	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	To facilitate networked discovery and information retrieval in the biomedical domain , we have designed a system for automatic assignment of Medical Subject Headings to documents retrieved from the World-Wide Web .
	manualset3
188224	4	415433	7	NULL	NULL	0	NULL	system	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	To facilitate networked discovery and information retrieval in the biomedical domain , we have designed a system for automatic assignment of Medical Subject Headings to documents retrieved from the World-Wide Web .
	manualset3
188225	5	415433	7	NULL	NULL	0	NULL	automatic assignment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To facilitate networked discovery and information retrieval in the biomedical domain , we have designed a system for automatic assignment of Medical Subject Headings to documents retrieved from the World-Wide Web .
	manualset3
188226	6	415433	7	NULL	NULL	0	NULL	Medical Subject Headings	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	To facilitate networked discovery and information retrieval in the biomedical domain , we have designed a system for automatic assignment of Medical Subject Headings to documents retrieved from the World-Wide Web .
	manualset3
188227	7	415433	7	NULL	NULL	0	NULL	documents	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	To facilitate networked discovery and information retrieval in the biomedical domain , we have designed a system for automatic assignment of Medical Subject Headings to documents retrieved from the World-Wide Web .
	manualset3
188228	8	415433	7	NULL	NULL	0	NULL	World-Wide Web	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	To facilitate networked discovery and information retrieval in the biomedical domain , we have designed a system for automatic assignment of Medical Subject Headings to documents retrieved from the World-Wide Web .
	manualset3
188229	1	415434	7	NULL	NULL	0	NULL	inclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To facilitate the inclusion of imperfect detection of individuals in such studies , we develop a method to estimate additive genetic variance and assess heritability for binary traits such as survival , using capture-recapture ( CR ) data .
	manualset3
188230	2	415434	7	NULL	NULL	0	NULL	 imperfect detection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To facilitate the inclusion of imperfect detection of individuals in such studies , we develop a method to estimate additive genetic variance and assess heritability for binary traits such as survival , using capture-recapture ( CR ) data .
	manualset3
188231	3	415434	7	NULL	NULL	0	NULL	individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To facilitate the inclusion of imperfect detection of individuals in such studies , we develop a method to estimate additive genetic variance and assess heritability for binary traits such as survival , using capture-recapture ( CR ) data .
	manualset3
188232	4	415434	7	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To facilitate the inclusion of imperfect detection of individuals in such studies , we develop a method to estimate additive genetic variance and assess heritability for binary traits such as survival , using capture-recapture ( CR ) data .
	manualset3
188233	5	415434	7	NULL	NULL	0	NULL	method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To facilitate the inclusion of imperfect detection of individuals in such studies , we develop a method to estimate additive genetic variance and assess heritability for binary traits such as survival , using capture-recapture ( CR ) data .
	manualset3
188234	6	415434	7	NULL	NULL	0	NULL	additive genetic variance	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	To facilitate the inclusion of imperfect detection of individuals in such studies , we develop a method to estimate additive genetic variance and assess heritability for binary traits such as survival , using capture-recapture ( CR ) data .
	manualset3
188235	7	415434	7	NULL	NULL	0	NULL	heritability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To facilitate the inclusion of imperfect detection of individuals in such studies , we develop a method to estimate additive genetic variance and assess heritability for binary traits such as survival , using capture-recapture ( CR ) data .
	manualset3
188236	8	415434	7	NULL	NULL	0	NULL	binary traits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To facilitate the inclusion of imperfect detection of individuals in such studies , we develop a method to estimate additive genetic variance and assess heritability for binary traits such as survival , using capture-recapture ( CR ) data .
	manualset3
188237	9	415434	7	NULL	NULL	0	NULL	survival 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To facilitate the inclusion of imperfect detection of individuals in such studies , we develop a method to estimate additive genetic variance and assess heritability for binary traits such as survival , using capture-recapture ( CR ) data .
	manualset3
188238	10	415434	7	NULL	NULL	0	NULL	capture-recapture ( CR ) data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	To facilitate the inclusion of imperfect detection of individuals in such studies , we develop a method to estimate additive genetic variance and assess heritability for binary traits such as survival , using capture-recapture ( CR ) data .
	manualset3
188239	1	415435	7	NULL	NULL	0	NULL	findings 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To follow up these findings suggesting involvement of a humoral factor , we incubated epitrochlearis muscles in serum before and during contractile activity in vitro .
	manualset3
188240	2	415435	7	NULL	NULL	NULL	NULL	humoral factor	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To follow up these findings suggesting involvement of a humoral factor , we incubated epitrochlearis muscles in serum before and during contractile activity in vitro .
	manualset3
188241	3	415435	7	NULL	NULL	0	NULL	epitrochlearis muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To follow up these findings suggesting involvement of a humoral factor , we incubated epitrochlearis muscles in serum before and during contractile activity in vitro .
	manualset3
188242	4	415435	7	NULL	NULL	0	NULL	serum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To follow up these findings suggesting involvement of a humoral factor , we incubated epitrochlearis muscles in serum before and during contractile activity in vitro .
	manualset3
188243	5	415435	7	NULL	NULL	0	NULL	contractile activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To follow up these findings suggesting involvement of a humoral factor , we incubated epitrochlearis muscles in serum before and during contractile activity in vitro .
	manualset3
188244	6	415435	7	NULL	NULL	0	NULL	involvement	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To follow up these findings suggesting involvement of a humoral factor , we incubated epitrochlearis muscles in serum before and during contractile activity in vitro .
	manualset3
188245	1	415436	7	NULL	NULL	0	NULL	active site 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	To further characterize the active site of gamma-secretase , we prepared a series of difluoro ketone peptide analogs with varying steric bulkiness in the P1 position and tested the ability of these compounds to inhibit Abeta production in APP-transfected cells .
	manualset3
188246	2	415436	7	NULL	NULL	0	NULL	gamma-secretase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To further characterize the active site of gamma-secretase , we prepared a series of difluoro ketone peptide analogs with varying steric bulkiness in the P1 position and tested the ability of these compounds to inhibit Abeta production in APP-transfected cells .
	manualset3
188247	3	415436	7	NULL	NULL	0	NULL	series	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To further characterize the active site of gamma-secretase , we prepared a series of difluoro ketone peptide analogs with varying steric bulkiness in the P1 position and tested the ability of these compounds to inhibit Abeta production in APP-transfected cells .
	manualset3
188248	4	415436	7	NULL	NULL	0	NULL	difluoro ketone peptide analogs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To further characterize the active site of gamma-secretase , we prepared a series of difluoro ketone peptide analogs with varying steric bulkiness in the P1 position and tested the ability of these compounds to inhibit Abeta production in APP-transfected cells .
	manualset3
188249	5	415436	7	NULL	NULL	0	NULL	steric bulkiness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To further characterize the active site of gamma-secretase , we prepared a series of difluoro ketone peptide analogs with varying steric bulkiness in the P1 position and tested the ability of these compounds to inhibit Abeta production in APP-transfected cells .
	manualset3
188250	6	415436	7	NULL	NULL	0	NULL	P1 position	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To further characterize the active site of gamma-secretase , we prepared a series of difluoro ketone peptide analogs with varying steric bulkiness in the P1 position and tested the ability of these compounds to inhibit Abeta production in APP-transfected cells .
	manualset3
188251	7	415436	7	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To further characterize the active site of gamma-secretase , we prepared a series of difluoro ketone peptide analogs with varying steric bulkiness in the P1 position and tested the ability of these compounds to inhibit Abeta production in APP-transfected cells .
	manualset3
188252	8	415436	7	NULL	NULL	0	NULL	compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To further characterize the active site of gamma-secretase , we prepared a series of difluoro ketone peptide analogs with varying steric bulkiness in the P1 position and tested the ability of these compounds to inhibit Abeta production in APP-transfected cells .
	manualset3
188253	9	415436	7	NULL	NULL	0	NULL	Abeta production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To further characterize the active site of gamma-secretase , we prepared a series of difluoro ketone peptide analogs with varying steric bulkiness in the P1 position and tested the ability of these compounds to inhibit Abeta production in APP-transfected cells .
	manualset3
188254	10	415436	7	NULL	NULL	0	NULL	APP-transfected cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To further characterize the active site of gamma-secretase , we prepared a series of difluoro ketone peptide analogs with varying steric bulkiness in the P1 position and tested the ability of these compounds to inhibit Abeta production in APP-transfected cells .
	manualset3
188282	1	415437	7	NULL	NULL	0	NULL	function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To further define the function of in malignant progression , we employed the small interference RNA ( siRNA ) technique to knockdown gene expression of TKTL1 in the gastric cancer cell line AGS .
	manualset3
188283	2	415437	7	NULL	NULL	0	NULL	malignant progression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To further define the function of in malignant progression , we employed the small interference RNA ( siRNA ) technique to knockdown gene expression of TKTL1 in the gastric cancer cell line AGS .
	manualset3
188284	3	415437	7	NULL	NULL	0	NULL	small interference RNA ( siRNA ) technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To further define the function of in malignant progression , we employed the small interference RNA ( siRNA ) technique to knockdown gene expression of TKTL1 in the gastric cancer cell line AGS .
	manualset3
188285	4	415437	7	NULL	NULL	0	NULL	gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To further define the function of in malignant progression , we employed the small interference RNA ( siRNA ) technique to knockdown gene expression of TKTL1 in the gastric cancer cell line AGS .
	manualset3
188286	5	415437	7	NULL	NULL	0	NULL	TKTL1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	To further define the function of in malignant progression , we employed the small interference RNA ( siRNA ) technique to knockdown gene expression of TKTL1 in the gastric cancer cell line AGS .
	manualset3
188287	6	415437	7	NULL	NULL	0	NULL	gastric cancer cell line 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To further define the function of in malignant progression , we employed the small interference RNA ( siRNA ) technique to knockdown gene expression of TKTL1 in the gastric cancer cell line AGS .
	manualset3
188288	7	415437	7	NULL	NULL	0	NULL	AGS 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To further define the function of in malignant progression , we employed the small interference RNA ( siRNA ) technique to knockdown gene expression of TKTL1 in the gastric cancer cell line AGS .
	manualset3
188289	1	415438	7	NULL	NULL	0	NULL	activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To further investigate the activity of serotonin neurons in relation to feeding behavior , the metabolic activity of the serotonergic system and single neuron activity changes in the lateral hypothalamic area ( LHA ) were investigated concurrently in freely behaving rats .
	manualset3
188290	2	415438	7	NULL	NULL	0	NULL	serotonin neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To further investigate the activity of serotonin neurons in relation to feeding behavior , the metabolic activity of the serotonergic system and single neuron activity changes in the lateral hypothalamic area ( LHA ) were investigated concurrently in freely behaving rats .
	manualset3
188291	3	415438	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	To further investigate the activity of serotonin neurons in relation to feeding behavior , the metabolic activity of the serotonergic system and single neuron activity changes in the lateral hypothalamic area ( LHA ) were investigated concurrently in freely behaving rats .
	manualset3
188292	4	415438	7	NULL	NULL	0	NULL	feeding behavior	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To further investigate the activity of serotonin neurons in relation to feeding behavior , the metabolic activity of the serotonergic system and single neuron activity changes in the lateral hypothalamic area ( LHA ) were investigated concurrently in freely behaving rats .
	manualset3
188293	5	415438	7	NULL	NULL	0	NULL	metabolic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To further investigate the activity of serotonin neurons in relation to feeding behavior , the metabolic activity of the serotonergic system and single neuron activity changes in the lateral hypothalamic area ( LHA ) were investigated concurrently in freely behaving rats .
	manualset3
188294	6	415438	7	NULL	NULL	0	NULL	serotonergic system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To further investigate the activity of serotonin neurons in relation to feeding behavior , the metabolic activity of the serotonergic system and single neuron activity changes in the lateral hypothalamic area ( LHA ) were investigated concurrently in freely behaving rats .
	manualset3
188295	7	415438	7	NULL	NULL	NULL	NULL	single neuron activity changes	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To further investigate the activity of serotonin neurons in relation to feeding behavior , the metabolic activity of the serotonergic system and single neuron activity changes in the lateral hypothalamic area ( LHA ) were investigated concurrently in freely behaving rats .
	manualset3
188296	8	415438	7	NULL	NULL	0	NULL	ateral hypothalamic area ( LHA ) 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To further investigate the activity of serotonin neurons in relation to feeding behavior , the metabolic activity of the serotonergic system and single neuron activity changes in the lateral hypothalamic area ( LHA ) were investigated concurrently in freely behaving rats .
	manualset3
188297	9	415438	7	NULL	NULL	0	NULL	freely behaving rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To further investigate the activity of serotonin neurons in relation to feeding behavior , the metabolic activity of the serotonergic system and single neuron activity changes in the lateral hypothalamic area ( LHA ) were investigated concurrently in freely behaving rats .
	manualset3
188298	1	415439	7	NULL	NULL	0	NULL	possibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To further investigate this possibility , wild-type and vitamin-C-deficient Arabidopsis thaliana ( L. ) Heynh ( vtc ) plants were transformed with a 35S : GLOase construct , homozygous lines were developed , and vitamin C levels were compared to those in untransformed controls .
	manualset3
188299	2	415439	7	NULL	NULL	0	NULL	wild-type  Arabidopsis thaliana ( L. ) Heynh ( vtc ) plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To further investigate this possibility , wild-type and vitamin-C-deficient Arabidopsis thaliana ( L. ) Heynh ( vtc ) plants were transformed with a 35S : GLOase construct , homozygous lines were developed , and vitamin C levels were compared to those in untransformed controls .
	manualset3
188300	3	415439	7	NULL	NULL	0	NULL	vitamin-C-deficient Arabidopsis thaliana ( L. ) Heynh ( vtc ) plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To further investigate this possibility , wild-type and vitamin-C-deficient Arabidopsis thaliana ( L. ) Heynh ( vtc ) plants were transformed with a 35S : GLOase construct , homozygous lines were developed , and vitamin C levels were compared to those in untransformed controls .
	manualset3
188301	4	415439	7	NULL	NULL	0	NULL	35S : GLOase construct	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To further investigate this possibility , wild-type and vitamin-C-deficient Arabidopsis thaliana ( L. ) Heynh ( vtc ) plants were transformed with a 35S : GLOase construct , homozygous lines were developed , and vitamin C levels were compared to those in untransformed controls .
	manualset3
188302	5	415439	7	NULL	NULL	0	NULL	homozygous lines 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To further investigate this possibility , wild-type and vitamin-C-deficient Arabidopsis thaliana ( L. ) Heynh ( vtc ) plants were transformed with a 35S : GLOase construct , homozygous lines were developed , and vitamin C levels were compared to those in untransformed controls .
	manualset3
188303	6	415439	7	NULL	NULL	0	NULL	vitamin C levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To further investigate this possibility , wild-type and vitamin-C-deficient Arabidopsis thaliana ( L. ) Heynh ( vtc ) plants were transformed with a 35S : GLOase construct , homozygous lines were developed , and vitamin C levels were compared to those in untransformed controls .
	manualset3
188304	7	415439	7	NULL	NULL	0	NULL	untransformed controls	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To further investigate this possibility , wild-type and vitamin-C-deficient Arabidopsis thaliana ( L. ) Heynh ( vtc ) plants were transformed with a 35S : GLOase construct , homozygous lines were developed , and vitamin C levels were compared to those in untransformed controls .
	manualset3
188305	1	415440	7	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To gain further insight into the role of FcgammaR polymorphisms in the genetic predisposition of SLE , association of FcgammaRIIa-H131R , IIb-I232T , IIIa-F176V and IIIb-NA1 / NA2 ( HNA-1a / 1b ) polymorphisms with SLE was analyzed in the Thai population , using case-control association analysis .
	manualset3
188306	2	415440	7	NULL	NULL	NULL	NULL	FcgammaR polymorphisms	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To gain further insight into the role of FcgammaR polymorphisms in the genetic predisposition of SLE , association of FcgammaRIIa-H131R , IIb-I232T , IIIa-F176V and IIIb-NA1 / NA2 ( HNA-1a / 1b ) polymorphisms with SLE was analyzed in the Thai population , using case-control association analysis .
	manualset3
188307	3	415440	7	NULL	NULL	0	NULL	genetic predisposition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To gain further insight into the role of FcgammaR polymorphisms in the genetic predisposition of SLE , association of FcgammaRIIa-H131R , IIb-I232T , IIIa-F176V and IIIb-NA1 / NA2 ( HNA-1a / 1b ) polymorphisms with SLE was analyzed in the Thai population , using case-control association analysis .
	manualset3
188308	4	415440	7	NULL	NULL	0	NULL	SLE	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To gain further insight into the role of FcgammaR polymorphisms in the genetic predisposition of SLE , association of FcgammaRIIa-H131R , IIb-I232T , IIIa-F176V and IIIb-NA1 / NA2 ( HNA-1a / 1b ) polymorphisms with SLE was analyzed in the Thai population , using case-control association analysis .
	manualset3
188309	5	415440	7	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	To gain further insight into the role of FcgammaR polymorphisms in the genetic predisposition of SLE , association of FcgammaRIIa-H131R , IIb-I232T , IIIa-F176V and IIIb-NA1 / NA2 ( HNA-1a / 1b ) polymorphisms with SLE was analyzed in the Thai population , using case-control association analysis .
	manualset3
188310	6	415440	7	NULL	NULL	NULL	NULL	FcgammaRIIa-H131R polymorphisms	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To gain further insight into the role of FcgammaR polymorphisms in the genetic predisposition of SLE , association of FcgammaRIIa-H131R , IIb-I232T , IIIa-F176V and IIIb-NA1 / NA2 ( HNA-1a / 1b ) polymorphisms with SLE was analyzed in the Thai population , using case-control association analysis .
	manualset3
188311	7	415440	7	NULL	NULL	NULL	NULL	IIb-I232T polymorphisms	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To gain further insight into the role of FcgammaR polymorphisms in the genetic predisposition of SLE , association of FcgammaRIIa-H131R , IIb-I232T , IIIa-F176V and IIIb-NA1 / NA2 ( HNA-1a / 1b ) polymorphisms with SLE was analyzed in the Thai population , using case-control association analysis .
	manualset3
188312	8	415440	7	NULL	NULL	NULL	NULL	 IIIa-F176V polymorphisms	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To gain further insight into the role of FcgammaR polymorphisms in the genetic predisposition of SLE , association of FcgammaRIIa-H131R , IIb-I232T , IIIa-F176V and IIIb-NA1 / NA2 ( HNA-1a / 1b ) polymorphisms with SLE was analyzed in the Thai population , using case-control association analysis .
	manualset3
188313	9	415440	7	NULL	NULL	NULL	NULL	IIIb-NA1 / NA2 polymorphisms	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To gain further insight into the role of FcgammaR polymorphisms in the genetic predisposition of SLE , association of FcgammaRIIa-H131R , IIb-I232T , IIIa-F176V and IIIb-NA1 / NA2 ( HNA-1a / 1b ) polymorphisms with SLE was analyzed in the Thai population , using case-control association analysis .
	manualset3
188314	10	415440	7	NULL	NULL	NULL	NULL	HNA-1a / 1b polymorphisms	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To gain further insight into the role of FcgammaR polymorphisms in the genetic predisposition of SLE , association of FcgammaRIIa-H131R , IIb-I232T , IIIa-F176V and IIIb-NA1 / NA2 ( HNA-1a / 1b ) polymorphisms with SLE was analyzed in the Thai population , using case-control association analysis .
	manualset3
188315	11	415440	7	NULL	NULL	0	NULL	SLE	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To gain further insight into the role of FcgammaR polymorphisms in the genetic predisposition of SLE , association of FcgammaRIIa-H131R , IIb-I232T , IIIa-F176V and IIIb-NA1 / NA2 ( HNA-1a / 1b ) polymorphisms with SLE was analyzed in the Thai population , using case-control association analysis .
	manualset3
188316	12	415440	7	NULL	NULL	0	NULL	Thai population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To gain further insight into the role of FcgammaR polymorphisms in the genetic predisposition of SLE , association of FcgammaRIIa-H131R , IIb-I232T , IIIa-F176V and IIIb-NA1 / NA2 ( HNA-1a / 1b ) polymorphisms with SLE was analyzed in the Thai population , using case-control association analysis .
	manualset3
188317	13	415440	7	NULL	NULL	0	NULL	case-control association analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To gain further insight into the role of FcgammaR polymorphisms in the genetic predisposition of SLE , association of FcgammaRIIa-H131R , IIb-I232T , IIIa-F176V and IIIb-NA1 / NA2 ( HNA-1a / 1b ) polymorphisms with SLE was analyzed in the Thai population , using case-control association analysis .
	manualset3
188318	1	415441	7	NULL	NULL	0	NULL	series	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After analyzing a series of protease inhibitors , we found E-64 , a specific thiol protease inhibitor , to be the most effective irreversible inhibitor of this enzyme , suggesting that the endoprotease might be a thiol protease .
	manualset3
188319	2	415441	7	NULL	NULL	0	NULL	protease inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After analyzing a series of protease inhibitors , we found E-64 , a specific thiol protease inhibitor , to be the most effective irreversible inhibitor of this enzyme , suggesting that the endoprotease might be a thiol protease .
	manualset3
188320	3	415441	7	NULL	NULL	0	NULL	E-64	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After analyzing a series of protease inhibitors , we found E-64 , a specific thiol protease inhibitor , to be the most effective irreversible inhibitor of this enzyme , suggesting that the endoprotease might be a thiol protease .
	manualset3
188321	4	415441	7	NULL	NULL	0	NULL	specific thiol protease inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After analyzing a series of protease inhibitors , we found E-64 , a specific thiol protease inhibitor , to be the most effective irreversible inhibitor of this enzyme , suggesting that the endoprotease might be a thiol protease .
	manualset3
188322	5	415441	7	NULL	NULL	0	NULL	irreversible inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After analyzing a series of protease inhibitors , we found E-64 , a specific thiol protease inhibitor , to be the most effective irreversible inhibitor of this enzyme , suggesting that the endoprotease might be a thiol protease .
	manualset3
188323	6	415441	7	NULL	NULL	0	NULL	enzyme	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	After analyzing a series of protease inhibitors , we found E-64 , a specific thiol protease inhibitor , to be the most effective irreversible inhibitor of this enzyme , suggesting that the endoprotease might be a thiol protease .
	manualset3
188324	7	415441	7	NULL	NULL	0	NULL	endoprotease	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	After analyzing a series of protease inhibitors , we found E-64 , a specific thiol protease inhibitor , to be the most effective irreversible inhibitor of this enzyme , suggesting that the endoprotease might be a thiol protease .
	manualset3
188325	8	415441	7	NULL	NULL	0	NULL	thiol protease	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	After analyzing a series of protease inhibitors , we found E-64 , a specific thiol protease inhibitor , to be the most effective irreversible inhibitor of this enzyme , suggesting that the endoprotease might be a thiol protease .
	manualset3
188358	1	415442	7	NULL	NULL	0	NULL	molecular events 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To gain insight into the molecular events occurring in the very early stages of barley microspore embryogenesis , cDNA clones corresponding to genes differentially expressed during the early stages of microspore culture were isolated and characterized .
	manualset3
188359	2	415442	7	NULL	NULL	0	NULL	very early stages	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To gain insight into the molecular events occurring in the very early stages of barley microspore embryogenesis , cDNA clones corresponding to genes differentially expressed during the early stages of microspore culture were isolated and characterized .
	manualset3
188362	3	415442	7	NULL	NULL	0	NULL	barley microspore embryogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To gain insight into the molecular events occurring in the very early stages of barley microspore embryogenesis , cDNA clones corresponding to genes differentially expressed during the early stages of microspore culture were isolated and characterized .
	manualset3
188365	4	415442	7	NULL	NULL	0	NULL	cDNA clones	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To gain insight into the molecular events occurring in the very early stages of barley microspore embryogenesis , cDNA clones corresponding to genes differentially expressed during the early stages of microspore culture were isolated and characterized .
	manualset3
188367	5	415442	7	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To gain insight into the molecular events occurring in the very early stages of barley microspore embryogenesis , cDNA clones corresponding to genes differentially expressed during the early stages of microspore culture were isolated and characterized .
	manualset3
188368	6	415442	7	NULL	NULL	0	NULL	early stages 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To gain insight into the molecular events occurring in the very early stages of barley microspore embryogenesis , cDNA clones corresponding to genes differentially expressed during the early stages of microspore culture were isolated and characterized .
	manualset3
188369	7	415442	7	NULL	NULL	0	NULL	microspore culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To gain insight into the molecular events occurring in the very early stages of barley microspore embryogenesis , cDNA clones corresponding to genes differentially expressed during the early stages of microspore culture were isolated and characterized .
	manualset3
188370	1	415443	7	NULL	NULL	0	NULL	cell adhesion molecules ( CAMs )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify cell adhesion molecules ( CAMs ) expressed by mammalian motoneurons , we applied the polymerase chain reaction to a murine motor neuron-like cell line , NSC-34 .
	manualset3
188371	2	415443	7	NULL	NULL	0	NULL	mammalian motoneurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify cell adhesion molecules ( CAMs ) expressed by mammalian motoneurons , we applied the polymerase chain reaction to a murine motor neuron-like cell line , NSC-34 .
	manualset3
188373	3	415443	7	NULL	NULL	0	NULL	Polymerase Chain Reaction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify cell adhesion molecules ( CAMs ) expressed by mammalian motoneurons , we applied the polymerase chain reaction to a murine motor neuron-like cell line , NSC-34 .
	manualset3
188375	4	415443	7	NULL	NULL	0	NULL	murine motor neuron-like cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify cell adhesion molecules ( CAMs ) expressed by mammalian motoneurons , we applied the polymerase chain reaction to a murine motor neuron-like cell line , NSC-34 .
	manualset3
188378	5	415443	7	NULL	NULL	0	NULL	NSC-34 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify cell adhesion molecules ( CAMs ) expressed by mammalian motoneurons , we applied the polymerase chain reaction to a murine motor neuron-like cell line , NSC-34 .
	manualset3
188382	1	415444	7	NULL	NULL	NULL	NULL	susceptibility variants 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To identify susceptibility variants for hepatitis B virus ( HBV ) - related hepatocellular carcinoma ( HCC ) , we conducted a genome-wide association study by genotyping 440 , 794 SNPs in 355 chronic HBV carriers with HCC and 360 chronic HBV carriers without HCC , all of Chinese ancestry .
	manualset3
188383	2	415444	7	NULL	NULL	0	NULL	hepatitis B virus ( HBV ) - related hepatocellular carcinoma ( HCC )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify susceptibility variants for hepatitis B virus ( HBV ) - related hepatocellular carcinoma ( HCC ) , we conducted a genome-wide association study by genotyping 440 , 794 SNPs in 355 chronic HBV carriers with HCC and 360 chronic HBV carriers without HCC , all of Chinese ancestry .
	manualset3
188384	3	415444	7	NULL	NULL	0	NULL	genome-wide association study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify susceptibility variants for hepatitis B virus ( HBV ) - related hepatocellular carcinoma ( HCC ) , we conducted a genome-wide association study by genotyping 440 , 794 SNPs in 355 chronic HBV carriers with HCC and 360 chronic HBV carriers without HCC , all of Chinese ancestry .
	manualset3
188385	4	415444	7	NULL	NULL	0	NULL	genotyping 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify susceptibility variants for hepatitis B virus ( HBV ) - related hepatocellular carcinoma ( HCC ) , we conducted a genome-wide association study by genotyping 440 , 794 SNPs in 355 chronic HBV carriers with HCC and 360 chronic HBV carriers without HCC , all of Chinese ancestry .
	manualset3
188386	5	415444	7	NULL	NULL	NULL	NULL	440 , 794 SNPs	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To identify susceptibility variants for hepatitis B virus ( HBV ) - related hepatocellular carcinoma ( HCC ) , we conducted a genome-wide association study by genotyping 440 , 794 SNPs in 355 chronic HBV carriers with HCC and 360 chronic HBV carriers without HCC , all of Chinese ancestry .
	manualset3
188388	7	415444	7	NULL	NULL	NULL	NULL	355 chronic HBV carriers	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To identify susceptibility variants for hepatitis B virus ( HBV ) - related hepatocellular carcinoma ( HCC ) , we conducted a genome-wide association study by genotyping 440 , 794 SNPs in 355 chronic HBV carriers with HCC and 360 chronic HBV carriers without HCC , all of Chinese ancestry .
	manualset3
188389	8	415444	7	NULL	NULL	0	NULL	HCC 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify susceptibility variants for hepatitis B virus ( HBV ) - related hepatocellular carcinoma ( HCC ) , we conducted a genome-wide association study by genotyping 440 , 794 SNPs in 355 chronic HBV carriers with HCC and 360 chronic HBV carriers without HCC , all of Chinese ancestry .
	manualset3
188390	9	415444	7	NULL	NULL	0	NULL	360 chronic HBV carriers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify susceptibility variants for hepatitis B virus ( HBV ) - related hepatocellular carcinoma ( HCC ) , we conducted a genome-wide association study by genotyping 440 , 794 SNPs in 355 chronic HBV carriers with HCC and 360 chronic HBV carriers without HCC , all of Chinese ancestry .
	manualset3
188391	10	415444	7	NULL	NULL	0	NULL	HCC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify susceptibility variants for hepatitis B virus ( HBV ) - related hepatocellular carcinoma ( HCC ) , we conducted a genome-wide association study by genotyping 440 , 794 SNPs in 355 chronic HBV carriers with HCC and 360 chronic HBV carriers without HCC , all of Chinese ancestry .
	manualset3
188392	11	415444	7	NULL	NULL	0	NULL	Chinese ancestry	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify susceptibility variants for hepatitis B virus ( HBV ) - related hepatocellular carcinoma ( HCC ) , we conducted a genome-wide association study by genotyping 440 , 794 SNPs in 355 chronic HBV carriers with HCC and 360 chronic HBV carriers without HCC , all of Chinese ancestry .
	manualset3
188393	1	415445	7	NULL	NULL	0	NULL	 characteristics	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify the characteristics of exemplary family physicians and consultants , we interviewed 25 family physicians and 25 consultants ( 5 each in the specialties of internal medicine , obstetrics and gynecology , pediatrics , psychiatry and surgery ) selected by their peers as being exemplary in their own practice setting .
	manualset3
188402	2	415445	7	NULL	NULL	0	NULL	exemplary family physicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify the characteristics of exemplary family physicians and consultants , we interviewed 25 family physicians and 25 consultants ( 5 each in the specialties of internal medicine , obstetrics and gynecology , pediatrics , psychiatry and surgery ) selected by their peers as being exemplary in their own practice setting .
	manualset3
188411	3	415445	7	NULL	NULL	0	NULL	consultants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify the characteristics of exemplary family physicians and consultants , we interviewed 25 family physicians and 25 consultants ( 5 each in the specialties of internal medicine , obstetrics and gynecology , pediatrics , psychiatry and surgery ) selected by their peers as being exemplary in their own practice setting .
	manualset3
188412	4	415445	7	NULL	NULL	0	NULL	25 family physicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify the characteristics of exemplary family physicians and consultants , we interviewed 25 family physicians and 25 consultants ( 5 each in the specialties of internal medicine , obstetrics and gynecology , pediatrics , psychiatry and surgery ) selected by their peers as being exemplary in their own practice setting .
	manualset3
188413	5	415445	7	NULL	NULL	0	NULL	25 consultants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify the characteristics of exemplary family physicians and consultants , we interviewed 25 family physicians and 25 consultants ( 5 each in the specialties of internal medicine , obstetrics and gynecology , pediatrics , psychiatry and surgery ) selected by their peers as being exemplary in their own practice setting .
	manualset3
188414	6	415445	7	NULL	NULL	0	NULL	5	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify the characteristics of exemplary family physicians and consultants , we interviewed 25 family physicians and 25 consultants ( 5 each in the specialties of internal medicine , obstetrics and gynecology , pediatrics , psychiatry and surgery ) selected by their peers as being exemplary in their own practice setting .
	manualset3
188415	7	415445	7	NULL	NULL	0	NULL	specialties	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify the characteristics of exemplary family physicians and consultants , we interviewed 25 family physicians and 25 consultants ( 5 each in the specialties of internal medicine , obstetrics and gynecology , pediatrics , psychiatry and surgery ) selected by their peers as being exemplary in their own practice setting .
	manualset3
188416	8	415445	7	NULL	NULL	0	NULL	internal medicine	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify the characteristics of exemplary family physicians and consultants , we interviewed 25 family physicians and 25 consultants ( 5 each in the specialties of internal medicine , obstetrics and gynecology , pediatrics , psychiatry and surgery ) selected by their peers as being exemplary in their own practice setting .
	manualset3
188417	9	415445	7	NULL	NULL	0	NULL	obstetrics and gynecology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify the characteristics of exemplary family physicians and consultants , we interviewed 25 family physicians and 25 consultants ( 5 each in the specialties of internal medicine , obstetrics and gynecology , pediatrics , psychiatry and surgery ) selected by their peers as being exemplary in their own practice setting .
	manualset3
188418	10	415445	7	NULL	NULL	0	NULL	pediatrics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify the characteristics of exemplary family physicians and consultants , we interviewed 25 family physicians and 25 consultants ( 5 each in the specialties of internal medicine , obstetrics and gynecology , pediatrics , psychiatry and surgery ) selected by their peers as being exemplary in their own practice setting .
	manualset3
188419	11	415445	7	NULL	NULL	0	NULL	psychiatry and surgery	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify the characteristics of exemplary family physicians and consultants , we interviewed 25 family physicians and 25 consultants ( 5 each in the specialties of internal medicine , obstetrics and gynecology , pediatrics , psychiatry and surgery ) selected by their peers as being exemplary in their own practice setting .
	manualset3
188420	12	415445	7	NULL	NULL	0	NULL	peers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify the characteristics of exemplary family physicians and consultants , we interviewed 25 family physicians and 25 consultants ( 5 each in the specialties of internal medicine , obstetrics and gynecology , pediatrics , psychiatry and surgery ) selected by their peers as being exemplary in their own practice setting .
	manualset3
188427	13	415445	7	NULL	NULL	NULL	NULL	practice setting	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To identify the characteristics of exemplary family physicians and consultants , we interviewed 25 family physicians and 25 consultants ( 5 each in the specialties of internal medicine , obstetrics and gynecology , pediatrics , psychiatry and surgery ) selected by their peers as being exemplary in their own practice setting .
	manualset3
188436	1	415446	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify the expression characteristics of these two genes , comparative mRNA analysis of nuc1 and nuc2 was carried out by quantitative real-time polymerase chain reaction ( PCR ) .
	manualset3
188437	2	415446	7	NULL	NULL	0	NULL	two genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify the expression characteristics of these two genes , comparative mRNA analysis of nuc1 and nuc2 was carried out by quantitative real-time polymerase chain reaction ( PCR ) .
	manualset3
188438	3	415446	7	NULL	NULL	0	NULL	comparative mRNA analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify the expression characteristics of these two genes , comparative mRNA analysis of nuc1 and nuc2 was carried out by quantitative real-time polymerase chain reaction ( PCR ) .
	manualset3
188439	4	415446	7	NULL	NULL	NULL	NULL	nuc1 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To identify the expression characteristics of these two genes , comparative mRNA analysis of nuc1 and nuc2 was carried out by quantitative real-time polymerase chain reaction ( PCR ) .
	manualset3
188440	5	415446	7	NULL	NULL	0	NULL	 nuc2	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify the expression characteristics of these two genes , comparative mRNA analysis of nuc1 and nuc2 was carried out by quantitative real-time polymerase chain reaction ( PCR ) .
	manualset3
188441	6	415446	7	NULL	NULL	0	NULL	quantitative real-time polymerase chain reaction ( PCR ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify the expression characteristics of these two genes , comparative mRNA analysis of nuc1 and nuc2 was carried out by quantitative real-time polymerase chain reaction ( PCR ) .
	manualset3
188452	1	415447	7	NULL	NULL	0	NULL	 mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify the mutations of fibrinogen genes in this family , all the exons and exon-intron boundaries of the three fibrinogen genes ( FGA , FGB , FGG ) were amplified by polymerase chain reaction , and direct sequencing of polymerase chain reaction products was performed , then the restriction endonuclease ( RsaI ) analysis was used to confirm the mutation .
	manualset3
188453	2	415447	7	NULL	NULL	NULL	NULL	fibrinogen genes 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To identify the mutations of fibrinogen genes in this family , all the exons and exon-intron boundaries of the three fibrinogen genes ( FGA , FGB , FGG ) were amplified by polymerase chain reaction , and direct sequencing of polymerase chain reaction products was performed , then the restriction endonuclease ( RsaI ) analysis was used to confirm the mutation .
	manualset3
188454	3	415447	7	NULL	NULL	0	NULL	family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify the mutations of fibrinogen genes in this family , all the exons and exon-intron boundaries of the three fibrinogen genes ( FGA , FGB , FGG ) were amplified by polymerase chain reaction , and direct sequencing of polymerase chain reaction products was performed , then the restriction endonuclease ( RsaI ) analysis was used to confirm the mutation .
	manualset3
188455	4	415447	7	NULL	NULL	0	NULL	exons	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify the mutations of fibrinogen genes in this family , all the exons and exon-intron boundaries of the three fibrinogen genes ( FGA , FGB , FGG ) were amplified by polymerase chain reaction , and direct sequencing of polymerase chain reaction products was performed , then the restriction endonuclease ( RsaI ) analysis was used to confirm the mutation .
	manualset3
188456	5	415447	7	NULL	NULL	0	NULL	exon-intron boundaries	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify the mutations of fibrinogen genes in this family , all the exons and exon-intron boundaries of the three fibrinogen genes ( FGA , FGB , FGG ) were amplified by polymerase chain reaction , and direct sequencing of polymerase chain reaction products was performed , then the restriction endonuclease ( RsaI ) analysis was used to confirm the mutation .
	manualset3
188457	6	415447	7	NULL	NULL	NULL	NULL	three fibrinogen genes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To identify the mutations of fibrinogen genes in this family , all the exons and exon-intron boundaries of the three fibrinogen genes ( FGA , FGB , FGG ) were amplified by polymerase chain reaction , and direct sequencing of polymerase chain reaction products was performed , then the restriction endonuclease ( RsaI ) analysis was used to confirm the mutation .
	manualset3
188458	7	415447	7	NULL	NULL	0	NULL	FGA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify the mutations of fibrinogen genes in this family , all the exons and exon-intron boundaries of the three fibrinogen genes ( FGA , FGB , FGG ) were amplified by polymerase chain reaction , and direct sequencing of polymerase chain reaction products was performed , then the restriction endonuclease ( RsaI ) analysis was used to confirm the mutation .
	manualset3
188459	8	415447	7	NULL	NULL	0	NULL	FGB	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify the mutations of fibrinogen genes in this family , all the exons and exon-intron boundaries of the three fibrinogen genes ( FGA , FGB , FGG ) were amplified by polymerase chain reaction , and direct sequencing of polymerase chain reaction products was performed , then the restriction endonuclease ( RsaI ) analysis was used to confirm the mutation .
	manualset3
188460	9	415447	7	NULL	NULL	0	NULL	FGG	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify the mutations of fibrinogen genes in this family , all the exons and exon-intron boundaries of the three fibrinogen genes ( FGA , FGB , FGG ) were amplified by polymerase chain reaction , and direct sequencing of polymerase chain reaction products was performed , then the restriction endonuclease ( RsaI ) analysis was used to confirm the mutation .
	manualset3
188461	10	415447	7	NULL	NULL	0	NULL	polymerase chain reaction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify the mutations of fibrinogen genes in this family , all the exons and exon-intron boundaries of the three fibrinogen genes ( FGA , FGB , FGG ) were amplified by polymerase chain reaction , and direct sequencing of polymerase chain reaction products was performed , then the restriction endonuclease ( RsaI ) analysis was used to confirm the mutation .
	manualset3
188462	11	415447	7	NULL	NULL	0	NULL	direct sequencing	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify the mutations of fibrinogen genes in this family , all the exons and exon-intron boundaries of the three fibrinogen genes ( FGA , FGB , FGG ) were amplified by polymerase chain reaction , and direct sequencing of polymerase chain reaction products was performed , then the restriction endonuclease ( RsaI ) analysis was used to confirm the mutation .
	manualset3
188463	12	415447	7	NULL	NULL	0	NULL	polymerase chain reaction products	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify the mutations of fibrinogen genes in this family , all the exons and exon-intron boundaries of the three fibrinogen genes ( FGA , FGB , FGG ) were amplified by polymerase chain reaction , and direct sequencing of polymerase chain reaction products was performed , then the restriction endonuclease ( RsaI ) analysis was used to confirm the mutation .
	manualset3
188464	13	415447	7	NULL	NULL	0	NULL	restriction endonuclease ( RsaI ) analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify the mutations of fibrinogen genes in this family , all the exons and exon-intron boundaries of the three fibrinogen genes ( FGA , FGB , FGG ) were amplified by polymerase chain reaction , and direct sequencing of polymerase chain reaction products was performed , then the restriction endonuclease ( RsaI ) analysis was used to confirm the mutation .
	manualset3
188465	14	415447	7	NULL	NULL	0	NULL	mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To identify the mutations of fibrinogen genes in this family , all the exons and exon-intron boundaries of the three fibrinogen genes ( FGA , FGB , FGG ) were amplified by polymerase chain reaction , and direct sequencing of polymerase chain reaction products was performed , then the restriction endonuclease ( RsaI ) analysis was used to confirm the mutation .
	manualset3
188496	1	415448	7	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To improve the ability of activated carbon felt-supported titanium dioxide ( TiO2/ACF ) to remove spores of P. expansum from the atmosphere , measurements for the removal efficiency of the spores at a temperature of 3 degrees C + / -1 degrees C and relative humidity of 90 % + / -3 % had been made on photocatalytically-activated ( PC ) silver-doped TiO2/ACF prepared by ion sputtering in two different modes and photoelectrocatalytically-activated ( PEC ) TiO2/ACF films .
	manualset3
188506	2	415448	7	NULL	NULL	0	NULL	activated carbon felt-supported titanium dioxide ( TiO2/ACF )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To improve the ability of activated carbon felt-supported titanium dioxide ( TiO2/ACF ) to remove spores of P. expansum from the atmosphere , measurements for the removal efficiency of the spores at a temperature of 3 degrees C + / -1 degrees C and relative humidity of 90 % + / -3 % had been made on photocatalytically-activated ( PC ) silver-doped TiO2/ACF prepared by ion sputtering in two different modes and photoelectrocatalytically-activated ( PEC ) TiO2/ACF films .
	manualset3
188509	3	415448	7	NULL	NULL	0	NULL	spores	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To improve the ability of activated carbon felt-supported titanium dioxide ( TiO2/ACF ) to remove spores of P. expansum from the atmosphere , measurements for the removal efficiency of the spores at a temperature of 3 degrees C + / -1 degrees C and relative humidity of 90 % + / -3 % had been made on photocatalytically-activated ( PC ) silver-doped TiO2/ACF prepared by ion sputtering in two different modes and photoelectrocatalytically-activated ( PEC ) TiO2/ACF films .
	manualset3
188510	4	415448	7	NULL	NULL	0	NULL	P. expansum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To improve the ability of activated carbon felt-supported titanium dioxide ( TiO2/ACF ) to remove spores of P. expansum from the atmosphere , measurements for the removal efficiency of the spores at a temperature of 3 degrees C + / -1 degrees C and relative humidity of 90 % + / -3 % had been made on photocatalytically-activated ( PC ) silver-doped TiO2/ACF prepared by ion sputtering in two different modes and photoelectrocatalytically-activated ( PEC ) TiO2/ACF films .
	manualset3
188511	5	415448	7	NULL	NULL	0	NULL	atmosphere	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	To improve the ability of activated carbon felt-supported titanium dioxide ( TiO2/ACF ) to remove spores of P. expansum from the atmosphere , measurements for the removal efficiency of the spores at a temperature of 3 degrees C + / -1 degrees C and relative humidity of 90 % + / -3 % had been made on photocatalytically-activated ( PC ) silver-doped TiO2/ACF prepared by ion sputtering in two different modes and photoelectrocatalytically-activated ( PEC ) TiO2/ACF films .
	manualset3
188512	6	415448	7	NULL	NULL	0	NULL	measurements	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	To improve the ability of activated carbon felt-supported titanium dioxide ( TiO2/ACF ) to remove spores of P. expansum from the atmosphere , measurements for the removal efficiency of the spores at a temperature of 3 degrees C + / -1 degrees C and relative humidity of 90 % + / -3 % had been made on photocatalytically-activated ( PC ) silver-doped TiO2/ACF prepared by ion sputtering in two different modes and photoelectrocatalytically-activated ( PEC ) TiO2/ACF films .
	manualset3
188516	7	415448	7	NULL	NULL	0	NULL	removal efficiency	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To improve the ability of activated carbon felt-supported titanium dioxide ( TiO2/ACF ) to remove spores of P. expansum from the atmosphere , measurements for the removal efficiency of the spores at a temperature of 3 degrees C + / -1 degrees C and relative humidity of 90 % + / -3 % had been made on photocatalytically-activated ( PC ) silver-doped TiO2/ACF prepared by ion sputtering in two different modes and photoelectrocatalytically-activated ( PEC ) TiO2/ACF films .
	manualset3
188522	8	415448	7	NULL	NULL	0	NULL	spores	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To improve the ability of activated carbon felt-supported titanium dioxide ( TiO2/ACF ) to remove spores of P. expansum from the atmosphere , measurements for the removal efficiency of the spores at a temperature of 3 degrees C + / -1 degrees C and relative humidity of 90 % + / -3 % had been made on photocatalytically-activated ( PC ) silver-doped TiO2/ACF prepared by ion sputtering in two different modes and photoelectrocatalytically-activated ( PEC ) TiO2/ACF films .
	manualset3
188524	9	415448	7	NULL	NULL	0	NULL	temperature	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To improve the ability of activated carbon felt-supported titanium dioxide ( TiO2/ACF ) to remove spores of P. expansum from the atmosphere , measurements for the removal efficiency of the spores at a temperature of 3 degrees C + / -1 degrees C and relative humidity of 90 % + / -3 % had been made on photocatalytically-activated ( PC ) silver-doped TiO2/ACF prepared by ion sputtering in two different modes and photoelectrocatalytically-activated ( PEC ) TiO2/ACF films .
	manualset3
188525	10	415448	7	NULL	NULL	0	NULL	3 degrees C + / -1 degrees C	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To improve the ability of activated carbon felt-supported titanium dioxide ( TiO2/ACF ) to remove spores of P. expansum from the atmosphere , measurements for the removal efficiency of the spores at a temperature of 3 degrees C + / -1 degrees C and relative humidity of 90 % + / -3 % had been made on photocatalytically-activated ( PC ) silver-doped TiO2/ACF prepared by ion sputtering in two different modes and photoelectrocatalytically-activated ( PEC ) TiO2/ACF films .
	manualset3
188526	11	415448	7	NULL	NULL	0	NULL	relative humidity	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	To improve the ability of activated carbon felt-supported titanium dioxide ( TiO2/ACF ) to remove spores of P. expansum from the atmosphere , measurements for the removal efficiency of the spores at a temperature of 3 degrees C + / -1 degrees C and relative humidity of 90 % + / -3 % had been made on photocatalytically-activated ( PC ) silver-doped TiO2/ACF prepared by ion sputtering in two different modes and photoelectrocatalytically-activated ( PEC ) TiO2/ACF films .
	manualset3
188528	12	415448	7	NULL	NULL	0	NULL	90 % + / -3 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	To improve the ability of activated carbon felt-supported titanium dioxide ( TiO2/ACF ) to remove spores of P. expansum from the atmosphere , measurements for the removal efficiency of the spores at a temperature of 3 degrees C + / -1 degrees C and relative humidity of 90 % + / -3 % had been made on photocatalytically-activated ( PC ) silver-doped TiO2/ACF prepared by ion sputtering in two different modes and photoelectrocatalytically-activated ( PEC ) TiO2/ACF films .
	manualset3
188531	13	415448	7	NULL	NULL	0	NULL	photocatalytically-activated ( PC ) silver-doped TiO2/ACF	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To improve the ability of activated carbon felt-supported titanium dioxide ( TiO2/ACF ) to remove spores of P. expansum from the atmosphere , measurements for the removal efficiency of the spores at a temperature of 3 degrees C + / -1 degrees C and relative humidity of 90 % + / -3 % had been made on photocatalytically-activated ( PC ) silver-doped TiO2/ACF prepared by ion sputtering in two different modes and photoelectrocatalytically-activated ( PEC ) TiO2/ACF films .
	manualset3
188534	14	415448	7	NULL	NULL	0	NULL	 ion sputtering	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To improve the ability of activated carbon felt-supported titanium dioxide ( TiO2/ACF ) to remove spores of P. expansum from the atmosphere , measurements for the removal efficiency of the spores at a temperature of 3 degrees C + / -1 degrees C and relative humidity of 90 % + / -3 % had been made on photocatalytically-activated ( PC ) silver-doped TiO2/ACF prepared by ion sputtering in two different modes and photoelectrocatalytically-activated ( PEC ) TiO2/ACF films .
	manualset3
188538	15	415448	7	NULL	NULL	NULL	NULL	two different modes	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To improve the ability of activated carbon felt-supported titanium dioxide ( TiO2/ACF ) to remove spores of P. expansum from the atmosphere , measurements for the removal efficiency of the spores at a temperature of 3 degrees C + / -1 degrees C and relative humidity of 90 % + / -3 % had been made on photocatalytically-activated ( PC ) silver-doped TiO2/ACF prepared by ion sputtering in two different modes and photoelectrocatalytically-activated ( PEC ) TiO2/ACF films .
	manualset3
188539	16	415448	7	NULL	NULL	NULL	NULL	photoelectrocatalytically-activated ( PEC ) TiO2/ACF films	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To improve the ability of activated carbon felt-supported titanium dioxide ( TiO2/ACF ) to remove spores of P. expansum from the atmosphere , measurements for the removal efficiency of the spores at a temperature of 3 degrees C + / -1 degrees C and relative humidity of 90 % + / -3 % had been made on photocatalytically-activated ( PC ) silver-doped TiO2/ACF prepared by ion sputtering in two different modes and photoelectrocatalytically-activated ( PEC ) TiO2/ACF films .
	manualset3
188545	1	415449	7	NULL	NULL	NULL	NULL	annealing	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After annealing at 490 C under Ar-flow , the polymer PAN is partially carbonized and the metallic nanoparticles are surrounded by a carbonaceous matrix .
	manualset3
188546	2	415449	7	NULL	NULL	0	NULL	490 C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	After annealing at 490 C under Ar-flow , the polymer PAN is partially carbonized and the metallic nanoparticles are surrounded by a carbonaceous matrix .
	manualset3
188547	3	415449	7	NULL	NULL	0	NULL	Ar-flow	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After annealing at 490 C under Ar-flow , the polymer PAN is partially carbonized and the metallic nanoparticles are surrounded by a carbonaceous matrix .
	manualset3
188551	4	415449	7	NULL	NULL	0	NULL	polymer PAN	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After annealing at 490 C under Ar-flow , the polymer PAN is partially carbonized and the metallic nanoparticles are surrounded by a carbonaceous matrix .
	manualset3
188552	5	415449	7	NULL	NULL	0	NULL	metallic nanoparticles	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	After annealing at 490 C under Ar-flow , the polymer PAN is partially carbonized and the metallic nanoparticles are surrounded by a carbonaceous matrix .
	manualset3
188553	6	415449	7	NULL	NULL	0	NULL	carbonaceous matrix	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After annealing at 490 C under Ar-flow , the polymer PAN is partially carbonized and the metallic nanoparticles are surrounded by a carbonaceous matrix .
	manualset3
188554	7	415449	7	NULL	NULL	0	NULL	partially carbonized	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After annealing at 490 C under Ar-flow , the polymer PAN is partially carbonized and the metallic nanoparticles are surrounded by a carbonaceous matrix .
	manualset3
188555	1	415450	7	NULL	NULL	0	NULL	 safety	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To improve the safety of plasma derived factor VIII ( FVIII ) concentrate , we introduced a final super heat treatment ( 100 degrees C for 30 min ) as additional virus inactivation step applied to a lyophilized , highly purified FVIII concentrate ( 100 IU/mg of proteins ) already virus inactivated using the solvent/detergent ( S/D ) method during the manufacturing process .
	manualset3
188556	2	415450	7	NULL	NULL	0	NULL	plasma derived factor VIII ( FVIII ) concentrate	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To improve the safety of plasma derived factor VIII ( FVIII ) concentrate , we introduced a final super heat treatment ( 100 degrees C for 30 min ) as additional virus inactivation step applied to a lyophilized , highly purified FVIII concentrate ( 100 IU/mg of proteins ) already virus inactivated using the solvent/detergent ( S/D ) method during the manufacturing process .
	manualset3
188557	3	415450	7	NULL	NULL	0	NULL	final super heat treatment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To improve the safety of plasma derived factor VIII ( FVIII ) concentrate , we introduced a final super heat treatment ( 100 degrees C for 30 min ) as additional virus inactivation step applied to a lyophilized , highly purified FVIII concentrate ( 100 IU/mg of proteins ) already virus inactivated using the solvent/detergent ( S/D ) method during the manufacturing process .
	manualset3
188558	4	415450	7	NULL	NULL	0	NULL	100 degrees C	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To improve the safety of plasma derived factor VIII ( FVIII ) concentrate , we introduced a final super heat treatment ( 100 degrees C for 30 min ) as additional virus inactivation step applied to a lyophilized , highly purified FVIII concentrate ( 100 IU/mg of proteins ) already virus inactivated using the solvent/detergent ( S/D ) method during the manufacturing process .
	manualset3
188559	5	415450	7	NULL	NULL	0	NULL	30 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	To improve the safety of plasma derived factor VIII ( FVIII ) concentrate , we introduced a final super heat treatment ( 100 degrees C for 30 min ) as additional virus inactivation step applied to a lyophilized , highly purified FVIII concentrate ( 100 IU/mg of proteins ) already virus inactivated using the solvent/detergent ( S/D ) method during the manufacturing process .
	manualset3
188560	6	415450	7	NULL	NULL	0	NULL	virus inactivation step	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To improve the safety of plasma derived factor VIII ( FVIII ) concentrate , we introduced a final super heat treatment ( 100 degrees C for 30 min ) as additional virus inactivation step applied to a lyophilized , highly purified FVIII concentrate ( 100 IU/mg of proteins ) already virus inactivated using the solvent/detergent ( S/D ) method during the manufacturing process .
	manualset3
188561	7	415450	7	NULL	NULL	0	NULL	lyophilized , highly purified FVIII concentrate	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To improve the safety of plasma derived factor VIII ( FVIII ) concentrate , we introduced a final super heat treatment ( 100 degrees C for 30 min ) as additional virus inactivation step applied to a lyophilized , highly purified FVIII concentrate ( 100 IU/mg of proteins ) already virus inactivated using the solvent/detergent ( S/D ) method during the manufacturing process .
	manualset3
188564	8	415450	7	NULL	NULL	0	NULL	100 IU/mg of proteins	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To improve the safety of plasma derived factor VIII ( FVIII ) concentrate , we introduced a final super heat treatment ( 100 degrees C for 30 min ) as additional virus inactivation step applied to a lyophilized , highly purified FVIII concentrate ( 100 IU/mg of proteins ) already virus inactivated using the solvent/detergent ( S/D ) method during the manufacturing process .
	manualset3
188567	9	415450	7	NULL	NULL	0	NULL	solvent/detergent ( S/D ) method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To improve the safety of plasma derived factor VIII ( FVIII ) concentrate , we introduced a final super heat treatment ( 100 degrees C for 30 min ) as additional virus inactivation step applied to a lyophilized , highly purified FVIII concentrate ( 100 IU/mg of proteins ) already virus inactivated using the solvent/detergent ( S/D ) method during the manufacturing process .
	manualset3
188569	10	415450	7	NULL	NULL	0	NULL	manufacturing process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To improve the safety of plasma derived factor VIII ( FVIII ) concentrate , we introduced a final super heat treatment ( 100 degrees C for 30 min ) as additional virus inactivation step applied to a lyophilized , highly purified FVIII concentrate ( 100 IU/mg of proteins ) already virus inactivated using the solvent/detergent ( S/D ) method during the manufacturing process .
	manualset3
188573	1	415451	7	NULL	NULL	0	NULL	 biocompatibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To increase biocompatibility , the poly-D-lysine ( PDL ) was immobilized on the SAMs ' modified microelectrodes .
	manualset3
188575	2	415451	7	NULL	NULL	0	NULL	poly-D-lysine ( PDL )	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To increase biocompatibility , the poly-D-lysine ( PDL ) was immobilized on the SAMs ' modified microelectrodes .
	manualset3
188577	3	415451	7	NULL	NULL	0	NULL	SAMs ' modified microelectrodes	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	To increase biocompatibility , the poly-D-lysine ( PDL ) was immobilized on the SAMs ' modified microelectrodes .
	manualset3
188581	1	415452	7	NULL	NULL	0	NULL	scope	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To increase its scope , the intervention may need to be tailored to the specific needs of groups that did not respond well to the intervention .
	manualset3
188583	2	415452	7	NULL	NULL	0	NULL	intervention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To increase its scope , the intervention may need to be tailored to the specific needs of groups that did not respond well to the intervention .
	manualset3
188584	3	415452	7	NULL	NULL	0	NULL	groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To increase its scope , the intervention may need to be tailored to the specific needs of groups that did not respond well to the intervention .
	manualset3
188585	4	415452	7	NULL	NULL	0	NULL	 intervention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To increase its scope , the intervention may need to be tailored to the specific needs of groups that did not respond well to the intervention .
	manualset3
191624	5	415452	7	NULL	NULL	0	NULL	specific needs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To increase its scope , the intervention may need to be tailored to the specific needs of groups that did not respond well to the intervention .
	manualset3
188589	1	415453	7	NULL	NULL	0	NULL	intracerebral inoculation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To intracerebral inoculation with JHM-CC virus , cortisone treated ICR mice survived without showing clinical signs , however , demyelinating lesions were produced in the brain and spinal cord of them .
	manualset3
188590	2	415453	7	NULL	NULL	0	NULL	JHM-CC virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To intracerebral inoculation with JHM-CC virus , cortisone treated ICR mice survived without showing clinical signs , however , demyelinating lesions were produced in the brain and spinal cord of them .
	manualset3
188592	3	415453	7	NULL	NULL	0	NULL	cortisone treated ICR mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To intracerebral inoculation with JHM-CC virus , cortisone treated ICR mice survived without showing clinical signs , however , demyelinating lesions were produced in the brain and spinal cord of them .
	manualset3
188593	4	415453	7	NULL	NULL	0	NULL	clinical signs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To intracerebral inoculation with JHM-CC virus , cortisone treated ICR mice survived without showing clinical signs , however , demyelinating lesions were produced in the brain and spinal cord of them .
	manualset3
188596	5	415453	7	NULL	NULL	0	NULL	demyelinating lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To intracerebral inoculation with JHM-CC virus , cortisone treated ICR mice survived without showing clinical signs , however , demyelinating lesions were produced in the brain and spinal cord of them .
	manualset3
188599	6	415453	7	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To intracerebral inoculation with JHM-CC virus , cortisone treated ICR mice survived without showing clinical signs , however , demyelinating lesions were produced in the brain and spinal cord of them .
	manualset3
188602	7	415453	7	NULL	NULL	0	NULL	spinal cord	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To intracerebral inoculation with JHM-CC virus , cortisone treated ICR mice survived without showing clinical signs , however , demyelinating lesions were produced in the brain and spinal cord of them .
	manualset3
188604	1	415454	7	NULL	NULL	NULL	NULL	basic visual information processing	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To investigate basic visual information processing in patients with hemineglect syndrome , pattern reversal visual evoked potentials ( VEPs ) were recorded in 21 brain-injured patients ( 10 with neglect symptoms ) and 6 healthy subjects .
	manualset3
188607	2	415454	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate basic visual information processing in patients with hemineglect syndrome , pattern reversal visual evoked potentials ( VEPs ) were recorded in 21 brain-injured patients ( 10 with neglect symptoms ) and 6 healthy subjects .
	manualset3
188610	3	415454	7	NULL	NULL	0	NULL	hemineglect syndrome 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate basic visual information processing in patients with hemineglect syndrome , pattern reversal visual evoked potentials ( VEPs ) were recorded in 21 brain-injured patients ( 10 with neglect symptoms ) and 6 healthy subjects .
	manualset3
188611	4	415454	7	NULL	NULL	0	NULL	pattern reversal visual evoked potentials ( VEPs )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate basic visual information processing in patients with hemineglect syndrome , pattern reversal visual evoked potentials ( VEPs ) were recorded in 21 brain-injured patients ( 10 with neglect symptoms ) and 6 healthy subjects .
	manualset3
188613	5	415454	7	NULL	NULL	0	NULL	21 brain-injured patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate basic visual information processing in patients with hemineglect syndrome , pattern reversal visual evoked potentials ( VEPs ) were recorded in 21 brain-injured patients ( 10 with neglect symptoms ) and 6 healthy subjects .
	manualset3
188615	6	415454	7	NULL	NULL	0	NULL	 10 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate basic visual information processing in patients with hemineglect syndrome , pattern reversal visual evoked potentials ( VEPs ) were recorded in 21 brain-injured patients ( 10 with neglect symptoms ) and 6 healthy subjects .
	manualset3
188616	7	415454	7	NULL	NULL	0	NULL	neglect symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate basic visual information processing in patients with hemineglect syndrome , pattern reversal visual evoked potentials ( VEPs ) were recorded in 21 brain-injured patients ( 10 with neglect symptoms ) and 6 healthy subjects .
	manualset3
188617	8	415454	7	NULL	NULL	0	NULL	6 healthy subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate basic visual information processing in patients with hemineglect syndrome , pattern reversal visual evoked potentials ( VEPs ) were recorded in 21 brain-injured patients ( 10 with neglect symptoms ) and 6 healthy subjects .
	manualset3
188618	1	415455	7	NULL	NULL	0	NULL	lung adenocarcinoma growth behavior	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate characteristic of lung adenocarcinoma growth behavior , we have established a cell line ( rat lung cancer in Nara ( RLCNR ) ) from a tumor induced by N-nitrosobis ( 2-hydroxypropyl ) amine ( BHP ) in a rat .
	manualset3
188621	2	415455	7	NULL	NULL	0	NULL	cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate characteristic of lung adenocarcinoma growth behavior , we have established a cell line ( rat lung cancer in Nara ( RLCNR ) ) from a tumor induced by N-nitrosobis ( 2-hydroxypropyl ) amine ( BHP ) in a rat .
	manualset3
188624	3	415455	7	NULL	NULL	0	NULL	rat lung cancer in Nara ( RLCNR )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate characteristic of lung adenocarcinoma growth behavior , we have established a cell line ( rat lung cancer in Nara ( RLCNR ) ) from a tumor induced by N-nitrosobis ( 2-hydroxypropyl ) amine ( BHP ) in a rat .
	manualset3
188626	4	415455	7	NULL	NULL	NULL	NULL	tumor	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To investigate characteristic of lung adenocarcinoma growth behavior , we have established a cell line ( rat lung cancer in Nara ( RLCNR ) ) from a tumor induced by N-nitrosobis ( 2-hydroxypropyl ) amine ( BHP ) in a rat .
	manualset3
188627	5	415455	7	NULL	NULL	0	NULL	N-nitrosobis ( 2-hydroxypropyl ) amine ( BHP )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate characteristic of lung adenocarcinoma growth behavior , we have established a cell line ( rat lung cancer in Nara ( RLCNR ) ) from a tumor induced by N-nitrosobis ( 2-hydroxypropyl ) amine ( BHP ) in a rat .
	manualset3
188628	6	415455	7	NULL	NULL	0	NULL	rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate characteristic of lung adenocarcinoma growth behavior , we have established a cell line ( rat lung cancer in Nara ( RLCNR ) ) from a tumor induced by N-nitrosobis ( 2-hydroxypropyl ) amine ( BHP ) in a rat .
	manualset3
188629	1	415456	7	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate further the activity and mechanism of action of PKCdelta , we have retrovirally transduced a PKCdelta cDNA in HCT116 human colon cancer cells .
	manualset3
188630	2	415456	7	NULL	NULL	0	NULL	mechanism of action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate further the activity and mechanism of action of PKCdelta , we have retrovirally transduced a PKCdelta cDNA in HCT116 human colon cancer cells .
	manualset3
188631	3	415456	7	NULL	NULL	NULL	NULL	PKCdelta	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To investigate further the activity and mechanism of action of PKCdelta , we have retrovirally transduced a PKCdelta cDNA in HCT116 human colon cancer cells .
	manualset3
188632	4	415456	7	NULL	NULL	0	NULL	PKCdelta cDNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate further the activity and mechanism of action of PKCdelta , we have retrovirally transduced a PKCdelta cDNA in HCT116 human colon cancer cells .
	manualset3
188633	5	415456	7	NULL	NULL	0	NULL	HCT116 human colon cancer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate further the activity and mechanism of action of PKCdelta , we have retrovirally transduced a PKCdelta cDNA in HCT116 human colon cancer cells .
	manualset3
188634	1	415457	7	NULL	NULL	0	NULL	 cGMP	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate how cGMP regulates ciliary activity , changes in ciliary beat frequency ( CBF ) and intracellular calcium concentration ( ( Ca2 + ) i ) of rabbit tracheal ciliated cells in response to 8-bromo-cGMP ( Br-cGMP ) were simultaneously quantified using digital , high-speed phase-contrast and fluorescence imaging .
	manualset3
188635	2	415457	7	NULL	NULL	0	NULL	ciliary activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate how cGMP regulates ciliary activity , changes in ciliary beat frequency ( CBF ) and intracellular calcium concentration ( ( Ca2 + ) i ) of rabbit tracheal ciliated cells in response to 8-bromo-cGMP ( Br-cGMP ) were simultaneously quantified using digital , high-speed phase-contrast and fluorescence imaging .
	manualset3
188636	3	415457	7	NULL	NULL	0	NULL	changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate how cGMP regulates ciliary activity , changes in ciliary beat frequency ( CBF ) and intracellular calcium concentration ( ( Ca2 + ) i ) of rabbit tracheal ciliated cells in response to 8-bromo-cGMP ( Br-cGMP ) were simultaneously quantified using digital , high-speed phase-contrast and fluorescence imaging .
	manualset3
188637	4	415457	7	NULL	NULL	0	NULL	ciliary beat frequency ( CBF ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate how cGMP regulates ciliary activity , changes in ciliary beat frequency ( CBF ) and intracellular calcium concentration ( ( Ca2 + ) i ) of rabbit tracheal ciliated cells in response to 8-bromo-cGMP ( Br-cGMP ) were simultaneously quantified using digital , high-speed phase-contrast and fluorescence imaging .
	manualset3
188638	5	415457	7	NULL	NULL	0	NULL	intracellular calcium concentration ( ( Ca2 + ) i )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate how cGMP regulates ciliary activity , changes in ciliary beat frequency ( CBF ) and intracellular calcium concentration ( ( Ca2 + ) i ) of rabbit tracheal ciliated cells in response to 8-bromo-cGMP ( Br-cGMP ) were simultaneously quantified using digital , high-speed phase-contrast and fluorescence imaging .
	manualset3
188639	6	415457	7	NULL	NULL	0	NULL	rabbit tracheal ciliated cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate how cGMP regulates ciliary activity , changes in ciliary beat frequency ( CBF ) and intracellular calcium concentration ( ( Ca2 + ) i ) of rabbit tracheal ciliated cells in response to 8-bromo-cGMP ( Br-cGMP ) were simultaneously quantified using digital , high-speed phase-contrast and fluorescence imaging .
	manualset3
188640	7	415457	7	NULL	NULL	0	NULL	8-bromo-cGMP ( Br-cGMP )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate how cGMP regulates ciliary activity , changes in ciliary beat frequency ( CBF ) and intracellular calcium concentration ( ( Ca2 + ) i ) of rabbit tracheal ciliated cells in response to 8-bromo-cGMP ( Br-cGMP ) were simultaneously quantified using digital , high-speed phase-contrast and fluorescence imaging .
	manualset3
188641	8	415457	7	NULL	NULL	0	NULL	digital , high-speed phase-contrast and fluorescence imaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate how cGMP regulates ciliary activity , changes in ciliary beat frequency ( CBF ) and intracellular calcium concentration ( ( Ca2 + ) i ) of rabbit tracheal ciliated cells in response to 8-bromo-cGMP ( Br-cGMP ) were simultaneously quantified using digital , high-speed phase-contrast and fluorescence imaging .
	manualset3
188646	1	415458	7	NULL	NULL	NULL	NULL	surface charge density effects	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To investigate surface charge density effects on adsorption of beta-Lg , the positive charge number per Au atom on the ( 100 ) surface , C , was varied from 0 to +0.0250 e .
	manualset3
188647	2	415458	7	NULL	NULL	NULL	NULL	adsorption	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To investigate surface charge density effects on adsorption of beta-Lg , the positive charge number per Au atom on the ( 100 ) surface , C , was varied from 0 to +0.0250 e .
	manualset3
188648	3	415458	7	NULL	NULL	0	NULL	beta-Lg	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate surface charge density effects on adsorption of beta-Lg , the positive charge number per Au atom on the ( 100 ) surface , C , was varied from 0 to +0.0250 e .
	manualset3
188649	4	415458	7	NULL	NULL	0	NULL	positive charge number per Au atom 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate surface charge density effects on adsorption of beta-Lg , the positive charge number per Au atom on the ( 100 ) surface , C , was varied from 0 to +0.0250 e .
	manualset3
188650	5	415458	7	NULL	NULL	0	NULL	( 100 ) surface	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate surface charge density effects on adsorption of beta-Lg , the positive charge number per Au atom on the ( 100 ) surface , C , was varied from 0 to +0.0250 e .
	manualset3
188651	6	415458	7	NULL	NULL	0	NULL	0 to +0.0250 e	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate surface charge density effects on adsorption of beta-Lg , the positive charge number per Au atom on the ( 100 ) surface , C , was varied from 0 to +0.0250 e .
	manualset3
188652	1	415459	7	NULL	NULL	0	NULL	cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the cause of accumulation of oxidised proteins in the livers of rats with carbon tetrachloride ( CCl4 ) induced liver cirrhosis , the activity of alkaline protease ( a high molecular weight , multisubunit cysteine proteinase ) was determined in the cirrhotic livers .
	manualset3
188653	2	415459	7	NULL	NULL	0	NULL	accumulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the cause of accumulation of oxidised proteins in the livers of rats with carbon tetrachloride ( CCl4 ) induced liver cirrhosis , the activity of alkaline protease ( a high molecular weight , multisubunit cysteine proteinase ) was determined in the cirrhotic livers .
	manualset3
188654	3	415459	7	NULL	NULL	0	NULL	oxidised proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the cause of accumulation of oxidised proteins in the livers of rats with carbon tetrachloride ( CCl4 ) induced liver cirrhosis , the activity of alkaline protease ( a high molecular weight , multisubunit cysteine proteinase ) was determined in the cirrhotic livers .
	manualset3
188657	4	415459	7	NULL	NULL	0	NULL	livers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the cause of accumulation of oxidised proteins in the livers of rats with carbon tetrachloride ( CCl4 ) induced liver cirrhosis , the activity of alkaline protease ( a high molecular weight , multisubunit cysteine proteinase ) was determined in the cirrhotic livers .
	manualset3
188658	5	415459	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the cause of accumulation of oxidised proteins in the livers of rats with carbon tetrachloride ( CCl4 ) induced liver cirrhosis , the activity of alkaline protease ( a high molecular weight , multisubunit cysteine proteinase ) was determined in the cirrhotic livers .
	manualset3
188659	6	415459	7	NULL	NULL	0	NULL	carbon tetrachloride ( CCl4 ) induced liver cirrhosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the cause of accumulation of oxidised proteins in the livers of rats with carbon tetrachloride ( CCl4 ) induced liver cirrhosis , the activity of alkaline protease ( a high molecular weight , multisubunit cysteine proteinase ) was determined in the cirrhotic livers .
	manualset3
188662	7	415459	7	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the cause of accumulation of oxidised proteins in the livers of rats with carbon tetrachloride ( CCl4 ) induced liver cirrhosis , the activity of alkaline protease ( a high molecular weight , multisubunit cysteine proteinase ) was determined in the cirrhotic livers .
	manualset3
188664	8	415459	7	NULL	NULL	0	NULL	alkaline protease	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the cause of accumulation of oxidised proteins in the livers of rats with carbon tetrachloride ( CCl4 ) induced liver cirrhosis , the activity of alkaline protease ( a high molecular weight , multisubunit cysteine proteinase ) was determined in the cirrhotic livers .
	manualset3
188667	9	415459	7	NULL	NULL	0	NULL	high molecular weight 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the cause of accumulation of oxidised proteins in the livers of rats with carbon tetrachloride ( CCl4 ) induced liver cirrhosis , the activity of alkaline protease ( a high molecular weight , multisubunit cysteine proteinase ) was determined in the cirrhotic livers .
	manualset3
188669	10	415459	7	NULL	NULL	0	NULL	multisubunit cysteine proteinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the cause of accumulation of oxidised proteins in the livers of rats with carbon tetrachloride ( CCl4 ) induced liver cirrhosis , the activity of alkaline protease ( a high molecular weight , multisubunit cysteine proteinase ) was determined in the cirrhotic livers .
	manualset3
188672	11	415459	7	NULL	NULL	0	NULL	cirrhotic livers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the cause of accumulation of oxidised proteins in the livers of rats with carbon tetrachloride ( CCl4 ) induced liver cirrhosis , the activity of alkaline protease ( a high molecular weight , multisubunit cysteine proteinase ) was determined in the cirrhotic livers .
	manualset3
188677	1	415460	7	NULL	NULL	0	NULL	effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the effect of the body temperature on muscle cell differentiation , we cultured the mouse myoblast cell lines C2C12 and Sol8 at lower temperatures than mouse body temperature .
	manualset3
188679	2	415460	7	NULL	NULL	0	NULL	body temperature 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the effect of the body temperature on muscle cell differentiation , we cultured the mouse myoblast cell lines C2C12 and Sol8 at lower temperatures than mouse body temperature .
	manualset3
188680	3	415460	7	NULL	NULL	0	NULL	muscle cell differentiation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the effect of the body temperature on muscle cell differentiation , we cultured the mouse myoblast cell lines C2C12 and Sol8 at lower temperatures than mouse body temperature .
	manualset3
188681	4	415460	7	NULL	NULL	0	NULL	mouse myoblast cell lines C2C12	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the effect of the body temperature on muscle cell differentiation , we cultured the mouse myoblast cell lines C2C12 and Sol8 at lower temperatures than mouse body temperature .
	manualset3
188683	5	415460	7	NULL	NULL	0	NULL	Sol8	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the effect of the body temperature on muscle cell differentiation , we cultured the mouse myoblast cell lines C2C12 and Sol8 at lower temperatures than mouse body temperature .
	manualset3
188686	6	415460	7	NULL	NULL	0	NULL	lower temperatures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the effect of the body temperature on muscle cell differentiation , we cultured the mouse myoblast cell lines C2C12 and Sol8 at lower temperatures than mouse body temperature .
	manualset3
188688	7	415460	7	NULL	NULL	0	NULL	mouse body temperature 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the effect of the body temperature on muscle cell differentiation , we cultured the mouse myoblast cell lines C2C12 and Sol8 at lower temperatures than mouse body temperature .
	manualset3
188691	1	415461	7	NULL	NULL	0	NULL	effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the effect of urotensin-II ( U-II ) on skin vascular tone in normotensive subjects and in patients with essential arterial hypertension ( EHT ) , forearm skin blood flux and skin blood flowmotion ( SBF ) response to U-II cathodal iontophoresis was investigated using laser Doppler flowmetry ( LDF ) and spectral Fourier analysis in 10 young normotensive subjects , before and after intra-dermal injection of the nitric oxide synthetase inhibitor N ( G ) - monometil-l-arginine ( L-NMMA ) .
	manualset3
188692	2	415461	7	NULL	NULL	0	NULL	urotensin-II ( U-II )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the effect of urotensin-II ( U-II ) on skin vascular tone in normotensive subjects and in patients with essential arterial hypertension ( EHT ) , forearm skin blood flux and skin blood flowmotion ( SBF ) response to U-II cathodal iontophoresis was investigated using laser Doppler flowmetry ( LDF ) and spectral Fourier analysis in 10 young normotensive subjects , before and after intra-dermal injection of the nitric oxide synthetase inhibitor N ( G ) - monometil-l-arginine ( L-NMMA ) .
	manualset3
188693	3	415461	7	NULL	NULL	0	NULL	skin vascular tone	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the effect of urotensin-II ( U-II ) on skin vascular tone in normotensive subjects and in patients with essential arterial hypertension ( EHT ) , forearm skin blood flux and skin blood flowmotion ( SBF ) response to U-II cathodal iontophoresis was investigated using laser Doppler flowmetry ( LDF ) and spectral Fourier analysis in 10 young normotensive subjects , before and after intra-dermal injection of the nitric oxide synthetase inhibitor N ( G ) - monometil-l-arginine ( L-NMMA ) .
	manualset3
188694	4	415461	7	NULL	NULL	0	NULL	normotensive subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the effect of urotensin-II ( U-II ) on skin vascular tone in normotensive subjects and in patients with essential arterial hypertension ( EHT ) , forearm skin blood flux and skin blood flowmotion ( SBF ) response to U-II cathodal iontophoresis was investigated using laser Doppler flowmetry ( LDF ) and spectral Fourier analysis in 10 young normotensive subjects , before and after intra-dermal injection of the nitric oxide synthetase inhibitor N ( G ) - monometil-l-arginine ( L-NMMA ) .
	manualset3
188695	5	415461	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the effect of urotensin-II ( U-II ) on skin vascular tone in normotensive subjects and in patients with essential arterial hypertension ( EHT ) , forearm skin blood flux and skin blood flowmotion ( SBF ) response to U-II cathodal iontophoresis was investigated using laser Doppler flowmetry ( LDF ) and spectral Fourier analysis in 10 young normotensive subjects , before and after intra-dermal injection of the nitric oxide synthetase inhibitor N ( G ) - monometil-l-arginine ( L-NMMA ) .
	manualset3
188696	6	415461	7	NULL	NULL	0	NULL	essential arterial hypertension ( EHT )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the effect of urotensin-II ( U-II ) on skin vascular tone in normotensive subjects and in patients with essential arterial hypertension ( EHT ) , forearm skin blood flux and skin blood flowmotion ( SBF ) response to U-II cathodal iontophoresis was investigated using laser Doppler flowmetry ( LDF ) and spectral Fourier analysis in 10 young normotensive subjects , before and after intra-dermal injection of the nitric oxide synthetase inhibitor N ( G ) - monometil-l-arginine ( L-NMMA ) .
	manualset3
188697	7	415461	7	NULL	NULL	0	NULL	forearm skin blood flux	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the effect of urotensin-II ( U-II ) on skin vascular tone in normotensive subjects and in patients with essential arterial hypertension ( EHT ) , forearm skin blood flux and skin blood flowmotion ( SBF ) response to U-II cathodal iontophoresis was investigated using laser Doppler flowmetry ( LDF ) and spectral Fourier analysis in 10 young normotensive subjects , before and after intra-dermal injection of the nitric oxide synthetase inhibitor N ( G ) - monometil-l-arginine ( L-NMMA ) .
	manualset3
188698	8	415461	7	NULL	NULL	0	NULL	skin blood flowmotion ( SBF ) response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the effect of urotensin-II ( U-II ) on skin vascular tone in normotensive subjects and in patients with essential arterial hypertension ( EHT ) , forearm skin blood flux and skin blood flowmotion ( SBF ) response to U-II cathodal iontophoresis was investigated using laser Doppler flowmetry ( LDF ) and spectral Fourier analysis in 10 young normotensive subjects , before and after intra-dermal injection of the nitric oxide synthetase inhibitor N ( G ) - monometil-l-arginine ( L-NMMA ) .
	manualset3
188699	9	415461	7	NULL	NULL	0	NULL	 U-II cathodal iontophoresis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the effect of urotensin-II ( U-II ) on skin vascular tone in normotensive subjects and in patients with essential arterial hypertension ( EHT ) , forearm skin blood flux and skin blood flowmotion ( SBF ) response to U-II cathodal iontophoresis was investigated using laser Doppler flowmetry ( LDF ) and spectral Fourier analysis in 10 young normotensive subjects , before and after intra-dermal injection of the nitric oxide synthetase inhibitor N ( G ) - monometil-l-arginine ( L-NMMA ) .
	manualset3
188700	10	415461	7	NULL	NULL	0	NULL	laser Doppler flowmetry ( LDF )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the effect of urotensin-II ( U-II ) on skin vascular tone in normotensive subjects and in patients with essential arterial hypertension ( EHT ) , forearm skin blood flux and skin blood flowmotion ( SBF ) response to U-II cathodal iontophoresis was investigated using laser Doppler flowmetry ( LDF ) and spectral Fourier analysis in 10 young normotensive subjects , before and after intra-dermal injection of the nitric oxide synthetase inhibitor N ( G ) - monometil-l-arginine ( L-NMMA ) .
	manualset3
188701	11	415461	7	NULL	NULL	0	NULL	spectral Fourier analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the effect of urotensin-II ( U-II ) on skin vascular tone in normotensive subjects and in patients with essential arterial hypertension ( EHT ) , forearm skin blood flux and skin blood flowmotion ( SBF ) response to U-II cathodal iontophoresis was investigated using laser Doppler flowmetry ( LDF ) and spectral Fourier analysis in 10 young normotensive subjects , before and after intra-dermal injection of the nitric oxide synthetase inhibitor N ( G ) - monometil-l-arginine ( L-NMMA ) .
	manualset3
188702	12	415461	7	NULL	NULL	0	NULL	10 young normotensive subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the effect of urotensin-II ( U-II ) on skin vascular tone in normotensive subjects and in patients with essential arterial hypertension ( EHT ) , forearm skin blood flux and skin blood flowmotion ( SBF ) response to U-II cathodal iontophoresis was investigated using laser Doppler flowmetry ( LDF ) and spectral Fourier analysis in 10 young normotensive subjects , before and after intra-dermal injection of the nitric oxide synthetase inhibitor N ( G ) - monometil-l-arginine ( L-NMMA ) .
	manualset3
188703	13	415461	7	NULL	NULL	0	NULL	intra-dermal injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the effect of urotensin-II ( U-II ) on skin vascular tone in normotensive subjects and in patients with essential arterial hypertension ( EHT ) , forearm skin blood flux and skin blood flowmotion ( SBF ) response to U-II cathodal iontophoresis was investigated using laser Doppler flowmetry ( LDF ) and spectral Fourier analysis in 10 young normotensive subjects , before and after intra-dermal injection of the nitric oxide synthetase inhibitor N ( G ) - monometil-l-arginine ( L-NMMA ) .
	manualset3
188704	14	415461	7	NULL	NULL	0	NULL	 nitric oxide synthetase inhibitor N ( G ) - monometil-l-arginine ( L-NMMA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the effect of urotensin-II ( U-II ) on skin vascular tone in normotensive subjects and in patients with essential arterial hypertension ( EHT ) , forearm skin blood flux and skin blood flowmotion ( SBF ) response to U-II cathodal iontophoresis was investigated using laser Doppler flowmetry ( LDF ) and spectral Fourier analysis in 10 young normotensive subjects , before and after intra-dermal injection of the nitric oxide synthetase inhibitor N ( G ) - monometil-l-arginine ( L-NMMA ) .
	manualset3
189011	1	415462	7	NULL	NULL	0	NULL	factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the factors that regulate eosinophil function in allergic airway disease , we have previously used segmental bronchoprovocation with allergen to study ex vivo eosinophil function .
	manualset3
189012	2	415462	7	NULL	NULL	0	NULL	 eosinophil function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the factors that regulate eosinophil function in allergic airway disease , we have previously used segmental bronchoprovocation with allergen to study ex vivo eosinophil function .
	manualset3
189013	3	415462	7	NULL	NULL	0	NULL	allergic airway disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the factors that regulate eosinophil function in allergic airway disease , we have previously used segmental bronchoprovocation with allergen to study ex vivo eosinophil function .
	manualset3
189014	4	415462	7	NULL	NULL	0	NULL	segmental bronchoprovocation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the factors that regulate eosinophil function in allergic airway disease , we have previously used segmental bronchoprovocation with allergen to study ex vivo eosinophil function .
	manualset3
189015	5	415462	7	NULL	NULL	0	NULL	allergen	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the factors that regulate eosinophil function in allergic airway disease , we have previously used segmental bronchoprovocation with allergen to study ex vivo eosinophil function .
	manualset3
189016	6	415462	7	NULL	NULL	0	NULL	ex vivo eosinophil function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the factors that regulate eosinophil function in allergic airway disease , we have previously used segmental bronchoprovocation with allergen to study ex vivo eosinophil function .
	manualset3
189017	1	415463	7	NULL	NULL	0	NULL	functional significance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the functional significance of this editing in vivo , we engineered mice deficient in GluR6 Q/R site editing .
	manualset3
189018	2	415463	7	NULL	NULL	0	NULL	editing 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the functional significance of this editing in vivo , we engineered mice deficient in GluR6 Q/R site editing .
	manualset3
189019	3	415463	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the functional significance of this editing in vivo , we engineered mice deficient in GluR6 Q/R site editing .
	manualset3
189020	4	415463	7	NULL	NULL	0	NULL	GluR6 Q/R site editing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the functional significance of this editing in vivo , we engineered mice deficient in GluR6 Q/R site editing .
	manualset3
189021	1	415464	7	NULL	NULL	0	NULL	 genetic association 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the genetic association of IL-7 / IL-7R signaling with the p53 pathway , we generated IL-7R ( null ) p53 ( null ) ( DKO ) mice .
	manualset3
189022	2	415464	7	NULL	NULL	0	NULL	IL-7 / IL-7R signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the genetic association of IL-7 / IL-7R signaling with the p53 pathway , we generated IL-7R ( null ) p53 ( null ) ( DKO ) mice .
	manualset3
189023	3	415464	7	NULL	NULL	0	NULL	p53 pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the genetic association of IL-7 / IL-7R signaling with the p53 pathway , we generated IL-7R ( null ) p53 ( null ) ( DKO ) mice .
	manualset3
189024	4	415464	7	NULL	NULL	0	NULL	IL-7R ( null ) p53 ( null ) ( DKO ) mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the genetic association of IL-7 / IL-7R signaling with the p53 pathway , we generated IL-7R ( null ) p53 ( null ) ( DKO ) mice .
	manualset3
189025	1	415465	7	NULL	NULL	0	NULL	 immunosuppressive effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the immunosuppressive effects of infectious bursal disease virus ( IBDV ) and aflatoxin in indigenous chickens of Uganda , Newcastle disease ( ND ) seronegative chicks were randomly allocated to two treatment groups .
	manualset3
189026	2	415465	7	NULL	NULL	0	NULL	infectious bursal disease virus ( IBDV ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the immunosuppressive effects of infectious bursal disease virus ( IBDV ) and aflatoxin in indigenous chickens of Uganda , Newcastle disease ( ND ) seronegative chicks were randomly allocated to two treatment groups .
	manualset3
189027	3	415465	7	NULL	NULL	0	NULL	aflatoxin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the immunosuppressive effects of infectious bursal disease virus ( IBDV ) and aflatoxin in indigenous chickens of Uganda , Newcastle disease ( ND ) seronegative chicks were randomly allocated to two treatment groups .
	manualset3
189028	4	415465	7	NULL	NULL	0	NULL	indigenous chickens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the immunosuppressive effects of infectious bursal disease virus ( IBDV ) and aflatoxin in indigenous chickens of Uganda , Newcastle disease ( ND ) seronegative chicks were randomly allocated to two treatment groups .
	manualset3
189029	5	415465	7	NULL	NULL	0	NULL	Uganda	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the immunosuppressive effects of infectious bursal disease virus ( IBDV ) and aflatoxin in indigenous chickens of Uganda , Newcastle disease ( ND ) seronegative chicks were randomly allocated to two treatment groups .
	manualset3
189030	6	415465	7	NULL	NULL	0	NULL	Newcastle disease ( ND ) seronegative chicks 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the immunosuppressive effects of infectious bursal disease virus ( IBDV ) and aflatoxin in indigenous chickens of Uganda , Newcastle disease ( ND ) seronegative chicks were randomly allocated to two treatment groups .
	manualset3
189031	7	415465	7	NULL	NULL	0	NULL	two treatment groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the immunosuppressive effects of infectious bursal disease virus ( IBDV ) and aflatoxin in indigenous chickens of Uganda , Newcastle disease ( ND ) seronegative chicks were randomly allocated to two treatment groups .
	manualset3
189032	1	415466	7	NULL	NULL	0	NULL	 lack	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the lack of O ( 2 ) inhibition of photosynthesis , we measured stromal and cytosolic fructose-1 , 6 - bisphosphatase , sucrose phosphate synthase , and partitioning of newly fixed carbon between starch and sucrose before , during , and after mild water stress .
	manualset3
189033	2	415466	7	NULL	NULL	0	NULL	 O ( 2 ) inhibition 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the lack of O ( 2 ) inhibition of photosynthesis , we measured stromal and cytosolic fructose-1 , 6 - bisphosphatase , sucrose phosphate synthase , and partitioning of newly fixed carbon between starch and sucrose before , during , and after mild water stress .
	manualset3
189034	3	415466	7	NULL	NULL	0	NULL	photosynthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the lack of O ( 2 ) inhibition of photosynthesis , we measured stromal and cytosolic fructose-1 , 6 - bisphosphatase , sucrose phosphate synthase , and partitioning of newly fixed carbon between starch and sucrose before , during , and after mild water stress .
	manualset3
189035	4	415466	7	NULL	NULL	0	NULL	stromal fructose-1 , 6 - bisphosphatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the lack of O ( 2 ) inhibition of photosynthesis , we measured stromal and cytosolic fructose-1 , 6 - bisphosphatase , sucrose phosphate synthase , and partitioning of newly fixed carbon between starch and sucrose before , during , and after mild water stress .
	manualset3
189036	5	415466	7	NULL	NULL	0	NULL	cytosolic fructose-1 , 6 - bisphosphatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the lack of O ( 2 ) inhibition of photosynthesis , we measured stromal and cytosolic fructose-1 , 6 - bisphosphatase , sucrose phosphate synthase , and partitioning of newly fixed carbon between starch and sucrose before , during , and after mild water stress .
	manualset3
189037	6	415466	7	NULL	NULL	0	NULL	sucrose phosphate synthase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the lack of O ( 2 ) inhibition of photosynthesis , we measured stromal and cytosolic fructose-1 , 6 - bisphosphatase , sucrose phosphate synthase , and partitioning of newly fixed carbon between starch and sucrose before , during , and after mild water stress .
	manualset3
189038	7	415466	7	NULL	NULL	0	NULL	partitioning 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the lack of O ( 2 ) inhibition of photosynthesis , we measured stromal and cytosolic fructose-1 , 6 - bisphosphatase , sucrose phosphate synthase , and partitioning of newly fixed carbon between starch and sucrose before , during , and after mild water stress .
	manualset3
189039	8	415466	7	NULL	NULL	0	NULL	newly fixed carbon	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the lack of O ( 2 ) inhibition of photosynthesis , we measured stromal and cytosolic fructose-1 , 6 - bisphosphatase , sucrose phosphate synthase , and partitioning of newly fixed carbon between starch and sucrose before , during , and after mild water stress .
	manualset3
189040	9	415466	7	NULL	NULL	0	NULL	starch 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the lack of O ( 2 ) inhibition of photosynthesis , we measured stromal and cytosolic fructose-1 , 6 - bisphosphatase , sucrose phosphate synthase , and partitioning of newly fixed carbon between starch and sucrose before , during , and after mild water stress .
	manualset3
189041	10	415466	7	NULL	NULL	0	NULL	sucrose	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the lack of O ( 2 ) inhibition of photosynthesis , we measured stromal and cytosolic fructose-1 , 6 - bisphosphatase , sucrose phosphate synthase , and partitioning of newly fixed carbon between starch and sucrose before , during , and after mild water stress .
	manualset3
189042	11	415466	7	NULL	NULL	0	NULL	mild water stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the lack of O ( 2 ) inhibition of photosynthesis , we measured stromal and cytosolic fructose-1 , 6 - bisphosphatase , sucrose phosphate synthase , and partitioning of newly fixed carbon between starch and sucrose before , during , and after mild water stress .
	manualset3
189043	1	415467	7	NULL	NULL	0	NULL	mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the mechanism of regulation of falcipain-2 by its prodomain , we expressed constructs encoding different portions of the prodomain and tested their ability to inhibit recombinant mature falcipain-2 .
	manualset3
189044	2	415467	7	NULL	NULL	0	NULL	regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the mechanism of regulation of falcipain-2 by its prodomain , we expressed constructs encoding different portions of the prodomain and tested their ability to inhibit recombinant mature falcipain-2 .
	manualset3
189045	3	415467	7	NULL	NULL	0	NULL	falcipain-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the mechanism of regulation of falcipain-2 by its prodomain , we expressed constructs encoding different portions of the prodomain and tested their ability to inhibit recombinant mature falcipain-2 .
	manualset3
189046	4	415467	7	NULL	NULL	0	NULL	prodomain 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the mechanism of regulation of falcipain-2 by its prodomain , we expressed constructs encoding different portions of the prodomain and tested their ability to inhibit recombinant mature falcipain-2 .
	manualset3
189047	5	415467	7	NULL	NULL	0	NULL	constructs	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the mechanism of regulation of falcipain-2 by its prodomain , we expressed constructs encoding different portions of the prodomain and tested their ability to inhibit recombinant mature falcipain-2 .
	manualset3
189048	6	415467	7	NULL	NULL	0	NULL	 different portions	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the mechanism of regulation of falcipain-2 by its prodomain , we expressed constructs encoding different portions of the prodomain and tested their ability to inhibit recombinant mature falcipain-2 .
	manualset3
189049	7	415467	7	NULL	NULL	0	NULL	prodomain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the mechanism of regulation of falcipain-2 by its prodomain , we expressed constructs encoding different portions of the prodomain and tested their ability to inhibit recombinant mature falcipain-2 .
	manualset3
189050	8	415467	7	NULL	NULL	0	NULL	ability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the mechanism of regulation of falcipain-2 by its prodomain , we expressed constructs encoding different portions of the prodomain and tested their ability to inhibit recombinant mature falcipain-2 .
	manualset3
189051	9	415467	7	NULL	NULL	0	NULL	recombinant mature falcipain-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the mechanism of regulation of falcipain-2 by its prodomain , we expressed constructs encoding different portions of the prodomain and tested their ability to inhibit recombinant mature falcipain-2 .
	manualset3
189052	1	415468	7	NULL	NULL	0	NULL	parS	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	After binding to parS , ParB spreads on the DNA , causing transcriptional silencing of nearby genes ( A. A. Bartosik et al. , J. Bacteriol .
	manualset3
189053	2	415468	7	NULL	NULL	0	NULL	ParB	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	After binding to parS , ParB spreads on the DNA , causing transcriptional silencing of nearby genes ( A. A. Bartosik et al. , J. Bacteriol .
	manualset3
189054	3	415468	7	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	After binding to parS , ParB spreads on the DNA , causing transcriptional silencing of nearby genes ( A. A. Bartosik et al. , J. Bacteriol .
	manualset3
189055	4	415468	7	NULL	NULL	0	NULL	transcriptional silencing 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After binding to parS , ParB spreads on the DNA , causing transcriptional silencing of nearby genes ( A. A. Bartosik et al. , J. Bacteriol .
	manualset3
189056	5	415468	7	NULL	NULL	NULL	NULL	nearby genes 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After binding to parS , ParB spreads on the DNA , causing transcriptional silencing of nearby genes ( A. A. Bartosik et al. , J. Bacteriol .
	manualset3
189057	6	415468	7	NULL	NULL	0	NULL	A. A. Bartosik et al. , J. Bacteriol .	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	After binding to parS , ParB spreads on the DNA , causing transcriptional silencing of nearby genes ( A. A. Bartosik et al. , J. Bacteriol .
	manualset3
191682	7	415468	7	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After binding to parS , ParB spreads on the DNA , causing transcriptional silencing of nearby genes ( A. A. Bartosik et al. , J. Bacteriol .
	manualset3
189058	1	415469	7	NULL	NULL	0	NULL	 mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the mechanisms responsible for the conversion of noradrenaline synthesizing precursors to adrenaline producing endocrine chromaffin cells we studied the role of glucocorticoids on the initial induction of adrenaline synthesis in embryonic adrenals and cultures of highly purified chromaffin precursor cells .
	manualset3
189059	2	415469	7	NULL	NULL	0	NULL	conversion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the mechanisms responsible for the conversion of noradrenaline synthesizing precursors to adrenaline producing endocrine chromaffin cells we studied the role of glucocorticoids on the initial induction of adrenaline synthesis in embryonic adrenals and cultures of highly purified chromaffin precursor cells .
	manualset3
189060	3	415469	7	NULL	NULL	0	NULL	noradrenaline synthesizing precursors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the mechanisms responsible for the conversion of noradrenaline synthesizing precursors to adrenaline producing endocrine chromaffin cells we studied the role of glucocorticoids on the initial induction of adrenaline synthesis in embryonic adrenals and cultures of highly purified chromaffin precursor cells .
	manualset3
189061	4	415469	7	NULL	NULL	0	NULL	adrenaline producing endocrine chromaffin cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the mechanisms responsible for the conversion of noradrenaline synthesizing precursors to adrenaline producing endocrine chromaffin cells we studied the role of glucocorticoids on the initial induction of adrenaline synthesis in embryonic adrenals and cultures of highly purified chromaffin precursor cells .
	manualset3
189062	5	415469	7	NULL	NULL	0	NULL	 role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the mechanisms responsible for the conversion of noradrenaline synthesizing precursors to adrenaline producing endocrine chromaffin cells we studied the role of glucocorticoids on the initial induction of adrenaline synthesis in embryonic adrenals and cultures of highly purified chromaffin precursor cells .
	manualset3
189063	6	415469	7	NULL	NULL	0	NULL	glucocorticoids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the mechanisms responsible for the conversion of noradrenaline synthesizing precursors to adrenaline producing endocrine chromaffin cells we studied the role of glucocorticoids on the initial induction of adrenaline synthesis in embryonic adrenals and cultures of highly purified chromaffin precursor cells .
	manualset3
189064	7	415469	7	NULL	NULL	0	NULL	initial induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the mechanisms responsible for the conversion of noradrenaline synthesizing precursors to adrenaline producing endocrine chromaffin cells we studied the role of glucocorticoids on the initial induction of adrenaline synthesis in embryonic adrenals and cultures of highly purified chromaffin precursor cells .
	manualset3
189065	8	415469	7	NULL	NULL	0	NULL	adrenaline synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the mechanisms responsible for the conversion of noradrenaline synthesizing precursors to adrenaline producing endocrine chromaffin cells we studied the role of glucocorticoids on the initial induction of adrenaline synthesis in embryonic adrenals and cultures of highly purified chromaffin precursor cells .
	manualset3
189066	9	415469	7	NULL	NULL	0	NULL	embryonic adrenals	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the mechanisms responsible for the conversion of noradrenaline synthesizing precursors to adrenaline producing endocrine chromaffin cells we studied the role of glucocorticoids on the initial induction of adrenaline synthesis in embryonic adrenals and cultures of highly purified chromaffin precursor cells .
	manualset3
189067	10	415469	7	NULL	NULL	0	NULL	cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the mechanisms responsible for the conversion of noradrenaline synthesizing precursors to adrenaline producing endocrine chromaffin cells we studied the role of glucocorticoids on the initial induction of adrenaline synthesis in embryonic adrenals and cultures of highly purified chromaffin precursor cells .
	manualset3
189068	11	415469	7	NULL	NULL	0	NULL	highly purified chromaffin precursor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the mechanisms responsible for the conversion of noradrenaline synthesizing precursors to adrenaline producing endocrine chromaffin cells we studied the role of glucocorticoids on the initial induction of adrenaline synthesis in embryonic adrenals and cultures of highly purified chromaffin precursor cells .
	manualset3
189069	1	415470	7	NULL	NULL	0	NULL	potential 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the potential of these molecules to provide protection against enteric infections when supplied orally , SIPs were generated against Transmissible gastroenteritis virus ( TGEV ) , a highly pathogenic porcine virus .
	manualset3
189070	2	415470	7	NULL	NULL	0	NULL	molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the potential of these molecules to provide protection against enteric infections when supplied orally , SIPs were generated against Transmissible gastroenteritis virus ( TGEV ) , a highly pathogenic porcine virus .
	manualset3
189071	3	415470	7	NULL	NULL	0	NULL	protection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the potential of these molecules to provide protection against enteric infections when supplied orally , SIPs were generated against Transmissible gastroenteritis virus ( TGEV ) , a highly pathogenic porcine virus .
	manualset3
189072	4	415470	7	NULL	NULL	0	NULL	enteric infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the potential of these molecules to provide protection against enteric infections when supplied orally , SIPs were generated against Transmissible gastroenteritis virus ( TGEV ) , a highly pathogenic porcine virus .
	manualset3
189073	5	415470	7	NULL	NULL	0	NULL	SIPs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the potential of these molecules to provide protection against enteric infections when supplied orally , SIPs were generated against Transmissible gastroenteritis virus ( TGEV ) , a highly pathogenic porcine virus .
	manualset3
189074	6	415470	7	NULL	NULL	0	NULL	Transmissible gastroenteritis virus ( TGEV ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the potential of these molecules to provide protection against enteric infections when supplied orally , SIPs were generated against Transmissible gastroenteritis virus ( TGEV ) , a highly pathogenic porcine virus .
	manualset3
189075	7	415470	7	NULL	NULL	0	NULL	highly pathogenic porcine virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the potential of these molecules to provide protection against enteric infections when supplied orally , SIPs were generated against Transmissible gastroenteritis virus ( TGEV ) , a highly pathogenic porcine virus .
	manualset3
189076	1	415471	7	NULL	NULL	0	NULL	 relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the relationship between forearm venous levels of catecholamines and systemic levels , simultaneous arterial and forearm vein blood samples were obtained from 14 subjects undergoing elective dental procedures and assayed with a sensitive and specific radioenzymatic assay .
	manualset3
189077	2	415471	7	NULL	NULL	0	NULL	forearm venous levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the relationship between forearm venous levels of catecholamines and systemic levels , simultaneous arterial and forearm vein blood samples were obtained from 14 subjects undergoing elective dental procedures and assayed with a sensitive and specific radioenzymatic assay .
	manualset3
189078	3	415471	7	NULL	NULL	0	NULL	catecholamines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the relationship between forearm venous levels of catecholamines and systemic levels , simultaneous arterial and forearm vein blood samples were obtained from 14 subjects undergoing elective dental procedures and assayed with a sensitive and specific radioenzymatic assay .
	manualset3
189079	4	415471	7	NULL	NULL	0	NULL	systemic levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the relationship between forearm venous levels of catecholamines and systemic levels , simultaneous arterial and forearm vein blood samples were obtained from 14 subjects undergoing elective dental procedures and assayed with a sensitive and specific radioenzymatic assay .
	manualset3
189080	5	415471	7	NULL	NULL	0	NULL	arterial blood samples	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the relationship between forearm venous levels of catecholamines and systemic levels , simultaneous arterial and forearm vein blood samples were obtained from 14 subjects undergoing elective dental procedures and assayed with a sensitive and specific radioenzymatic assay .
	manualset3
189081	6	415471	7	NULL	NULL	0	NULL	forearm vein blood samples	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the relationship between forearm venous levels of catecholamines and systemic levels , simultaneous arterial and forearm vein blood samples were obtained from 14 subjects undergoing elective dental procedures and assayed with a sensitive and specific radioenzymatic assay .
	manualset3
189082	7	415471	7	NULL	NULL	0	NULL	14 subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the relationship between forearm venous levels of catecholamines and systemic levels , simultaneous arterial and forearm vein blood samples were obtained from 14 subjects undergoing elective dental procedures and assayed with a sensitive and specific radioenzymatic assay .
	manualset3
189083	8	415471	7	NULL	NULL	0	NULL	elective dental procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the relationship between forearm venous levels of catecholamines and systemic levels , simultaneous arterial and forearm vein blood samples were obtained from 14 subjects undergoing elective dental procedures and assayed with a sensitive and specific radioenzymatic assay .
	manualset3
189084	9	415471	7	NULL	NULL	0	NULL	sensitive and specific radioenzymatic assay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the relationship between forearm venous levels of catecholamines and systemic levels , simultaneous arterial and forearm vein blood samples were obtained from 14 subjects undergoing elective dental procedures and assayed with a sensitive and specific radioenzymatic assay .
	manualset3
189085	1	415472	7	NULL	NULL	0	NULL	 role 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the role of interferon regulatory factors ( IRFs ) in inflammation-associated megakaryopoiesis , mouse bone marrow hematopoietic stem cells ( HSCs ) were analyzed .
	manualset3
189086	2	415472	7	NULL	NULL	0	NULL	interferon regulatory factors ( IRFs )	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the role of interferon regulatory factors ( IRFs ) in inflammation-associated megakaryopoiesis , mouse bone marrow hematopoietic stem cells ( HSCs ) were analyzed .
	manualset3
189087	3	415472	7	NULL	NULL	0	NULL	inflammation-associated megakaryopoiesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the role of interferon regulatory factors ( IRFs ) in inflammation-associated megakaryopoiesis , mouse bone marrow hematopoietic stem cells ( HSCs ) were analyzed .
	manualset3
189088	4	415472	7	NULL	NULL	0	NULL	mouse bone marrow hematopoietic stem cells ( HSCs )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the role of interferon regulatory factors ( IRFs ) in inflammation-associated megakaryopoiesis , mouse bone marrow hematopoietic stem cells ( HSCs ) were analyzed .
	manualset3
189089	1	415473	7	NULL	NULL	0	NULL	short - term effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the short - and long-term effects of axotomy on the survival of central nervous system ( CNS ) neurons in adult rats , retinal ganglion cells ( RGCs ) were labeled retrogradely with the persistent marker diI and their axons interrupted in the optic nerve ( ON ) by intracranial crush 8 or 10 mm from the eye or intraorbital cut 0.5 or 3 mm from the eye .
	manualset3
189090	2	415473	7	NULL	NULL	0	NULL	long-term effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the short - and long-term effects of axotomy on the survival of central nervous system ( CNS ) neurons in adult rats , retinal ganglion cells ( RGCs ) were labeled retrogradely with the persistent marker diI and their axons interrupted in the optic nerve ( ON ) by intracranial crush 8 or 10 mm from the eye or intraorbital cut 0.5 or 3 mm from the eye .
	manualset3
189091	3	415473	7	NULL	NULL	0	NULL	axotomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the short - and long-term effects of axotomy on the survival of central nervous system ( CNS ) neurons in adult rats , retinal ganglion cells ( RGCs ) were labeled retrogradely with the persistent marker diI and their axons interrupted in the optic nerve ( ON ) by intracranial crush 8 or 10 mm from the eye or intraorbital cut 0.5 or 3 mm from the eye .
	manualset3
189092	4	415473	7	NULL	NULL	0	NULL	survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the short - and long-term effects of axotomy on the survival of central nervous system ( CNS ) neurons in adult rats , retinal ganglion cells ( RGCs ) were labeled retrogradely with the persistent marker diI and their axons interrupted in the optic nerve ( ON ) by intracranial crush 8 or 10 mm from the eye or intraorbital cut 0.5 or 3 mm from the eye .
	manualset3
189093	5	415473	7	NULL	NULL	0	NULL	central nervous system ( CNS ) neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the short - and long-term effects of axotomy on the survival of central nervous system ( CNS ) neurons in adult rats , retinal ganglion cells ( RGCs ) were labeled retrogradely with the persistent marker diI and their axons interrupted in the optic nerve ( ON ) by intracranial crush 8 or 10 mm from the eye or intraorbital cut 0.5 or 3 mm from the eye .
	manualset3
189094	6	415473	7	NULL	NULL	0	NULL	adult rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the short - and long-term effects of axotomy on the survival of central nervous system ( CNS ) neurons in adult rats , retinal ganglion cells ( RGCs ) were labeled retrogradely with the persistent marker diI and their axons interrupted in the optic nerve ( ON ) by intracranial crush 8 or 10 mm from the eye or intraorbital cut 0.5 or 3 mm from the eye .
	manualset3
189095	7	415473	7	NULL	NULL	0	NULL	retinal ganglion cells ( RGCs )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the short - and long-term effects of axotomy on the survival of central nervous system ( CNS ) neurons in adult rats , retinal ganglion cells ( RGCs ) were labeled retrogradely with the persistent marker diI and their axons interrupted in the optic nerve ( ON ) by intracranial crush 8 or 10 mm from the eye or intraorbital cut 0.5 or 3 mm from the eye .
	manualset3
189096	8	415473	7	NULL	NULL	0	NULL	persistent marker diI	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the short - and long-term effects of axotomy on the survival of central nervous system ( CNS ) neurons in adult rats , retinal ganglion cells ( RGCs ) were labeled retrogradely with the persistent marker diI and their axons interrupted in the optic nerve ( ON ) by intracranial crush 8 or 10 mm from the eye or intraorbital cut 0.5 or 3 mm from the eye .
	manualset3
189097	9	415473	7	NULL	NULL	0	NULL	axons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the short - and long-term effects of axotomy on the survival of central nervous system ( CNS ) neurons in adult rats , retinal ganglion cells ( RGCs ) were labeled retrogradely with the persistent marker diI and their axons interrupted in the optic nerve ( ON ) by intracranial crush 8 or 10 mm from the eye or intraorbital cut 0.5 or 3 mm from the eye .
	manualset3
189098	10	415473	7	NULL	NULL	0	NULL	optic nerve ( ON )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the short - and long-term effects of axotomy on the survival of central nervous system ( CNS ) neurons in adult rats , retinal ganglion cells ( RGCs ) were labeled retrogradely with the persistent marker diI and their axons interrupted in the optic nerve ( ON ) by intracranial crush 8 or 10 mm from the eye or intraorbital cut 0.5 or 3 mm from the eye .
	manualset3
189099	11	415473	7	NULL	NULL	0	NULL	intracranial crush 8 or 10 mm	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the short - and long-term effects of axotomy on the survival of central nervous system ( CNS ) neurons in adult rats , retinal ganglion cells ( RGCs ) were labeled retrogradely with the persistent marker diI and their axons interrupted in the optic nerve ( ON ) by intracranial crush 8 or 10 mm from the eye or intraorbital cut 0.5 or 3 mm from the eye .
	manualset3
189100	12	415473	7	NULL	NULL	0	NULL	eye	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the short - and long-term effects of axotomy on the survival of central nervous system ( CNS ) neurons in adult rats , retinal ganglion cells ( RGCs ) were labeled retrogradely with the persistent marker diI and their axons interrupted in the optic nerve ( ON ) by intracranial crush 8 or 10 mm from the eye or intraorbital cut 0.5 or 3 mm from the eye .
	manualset3
189101	13	415473	7	NULL	NULL	0	NULL	 intraorbital cut 0.5 or 3 mm 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the short - and long-term effects of axotomy on the survival of central nervous system ( CNS ) neurons in adult rats , retinal ganglion cells ( RGCs ) were labeled retrogradely with the persistent marker diI and their axons interrupted in the optic nerve ( ON ) by intracranial crush 8 or 10 mm from the eye or intraorbital cut 0.5 or 3 mm from the eye .
	manualset3
189102	14	415473	7	NULL	NULL	0	NULL	 eye 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate the short - and long-term effects of axotomy on the survival of central nervous system ( CNS ) neurons in adult rats , retinal ganglion cells ( RGCs ) were labeled retrogradely with the persistent marker diI and their axons interrupted in the optic nerve ( ON ) by intracranial crush 8 or 10 mm from the eye or intraorbital cut 0.5 or 3 mm from the eye .
	manualset3
189103	1	415474	7	NULL	NULL	0	NULL	contributions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate these contributions , multimodal functional magnetic resonance imaging was employed to monitor responses of BOLD , cerebral blood flow ( CBF ) , total CBV , and arterial CBV ( CBV ( a ) ) in human visual cortex after brief breath hold and visual stimulation .
	manualset3
189104	2	415474	7	NULL	NULL	0	NULL	multimodal functional magnetic resonance imaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate these contributions , multimodal functional magnetic resonance imaging was employed to monitor responses of BOLD , cerebral blood flow ( CBF ) , total CBV , and arterial CBV ( CBV ( a ) ) in human visual cortex after brief breath hold and visual stimulation .
	manualset3
189105	3	415474	7	NULL	NULL	0	NULL	responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate these contributions , multimodal functional magnetic resonance imaging was employed to monitor responses of BOLD , cerebral blood flow ( CBF ) , total CBV , and arterial CBV ( CBV ( a ) ) in human visual cortex after brief breath hold and visual stimulation .
	manualset3
189106	4	415474	7	NULL	NULL	0	NULL	BOLD	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate these contributions , multimodal functional magnetic resonance imaging was employed to monitor responses of BOLD , cerebral blood flow ( CBF ) , total CBV , and arterial CBV ( CBV ( a ) ) in human visual cortex after brief breath hold and visual stimulation .
	manualset3
189107	5	415474	7	NULL	NULL	0	NULL	cerebral blood flow ( CBF ) 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate these contributions , multimodal functional magnetic resonance imaging was employed to monitor responses of BOLD , cerebral blood flow ( CBF ) , total CBV , and arterial CBV ( CBV ( a ) ) in human visual cortex after brief breath hold and visual stimulation .
	manualset3
189108	6	415474	7	NULL	NULL	0	NULL	total CBV	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate these contributions , multimodal functional magnetic resonance imaging was employed to monitor responses of BOLD , cerebral blood flow ( CBF ) , total CBV , and arterial CBV ( CBV ( a ) ) in human visual cortex after brief breath hold and visual stimulation .
	manualset3
189109	7	415474	7	NULL	NULL	0	NULL	arterial CBV ( CBV ( a ) )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate these contributions , multimodal functional magnetic resonance imaging was employed to monitor responses of BOLD , cerebral blood flow ( CBF ) , total CBV , and arterial CBV ( CBV ( a ) ) in human visual cortex after brief breath hold and visual stimulation .
	manualset3
189110	8	415474	7	NULL	NULL	0	NULL	human visual cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate these contributions , multimodal functional magnetic resonance imaging was employed to monitor responses of BOLD , cerebral blood flow ( CBF ) , total CBV , and arterial CBV ( CBV ( a ) ) in human visual cortex after brief breath hold and visual stimulation .
	manualset3
189111	9	415474	7	NULL	NULL	0	NULL	 visual stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate these contributions , multimodal functional magnetic resonance imaging was employed to monitor responses of BOLD , cerebral blood flow ( CBF ) , total CBV , and arterial CBV ( CBV ( a ) ) in human visual cortex after brief breath hold and visual stimulation .
	manualset3
189112	1	415475	7	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate this hypothesis we examined motor unit size with electrographic examinations in 14 patients ( six with mild TD ; eight without and all with psychotic illness ) .
	manualset3
189113	2	415475	7	NULL	NULL	0	NULL	motor unit size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate this hypothesis we examined motor unit size with electrographic examinations in 14 patients ( six with mild TD ; eight without and all with psychotic illness ) .
	manualset3
189114	3	415475	7	NULL	NULL	0	NULL	electrographic examinations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate this hypothesis we examined motor unit size with electrographic examinations in 14 patients ( six with mild TD ; eight without and all with psychotic illness ) .
	manualset3
189115	4	415475	7	NULL	NULL	0	NULL	14 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate this hypothesis we examined motor unit size with electrographic examinations in 14 patients ( six with mild TD ; eight without and all with psychotic illness ) .
	manualset3
189116	5	415475	7	NULL	NULL	0	NULL	six	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate this hypothesis we examined motor unit size with electrographic examinations in 14 patients ( six with mild TD ; eight without and all with psychotic illness ) .
	manualset3
189117	6	415475	7	NULL	NULL	0	NULL	mild TD	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate this hypothesis we examined motor unit size with electrographic examinations in 14 patients ( six with mild TD ; eight without and all with psychotic illness ) .
	manualset3
189118	7	415475	7	NULL	NULL	0	NULL	eight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate this hypothesis we examined motor unit size with electrographic examinations in 14 patients ( six with mild TD ; eight without and all with psychotic illness ) .
	manualset3
189119	8	415475	7	NULL	NULL	0	NULL	psychotic illness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate this hypothesis we examined motor unit size with electrographic examinations in 14 patients ( six with mild TD ; eight without and all with psychotic illness ) .
	manualset3
189120	1	415476	7	NULL	NULL	0	NULL	CD5 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate this we cloned the CD5 gene from a rabbit cosmid library , using a probe derived from human CD5 cDNA .
	manualset3
189121	2	415476	7	NULL	NULL	0	NULL	rabbit cosmid library	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate this we cloned the CD5 gene from a rabbit cosmid library , using a probe derived from human CD5 cDNA .
	manualset3
189122	3	415476	7	NULL	NULL	0	NULL	probe	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate this we cloned the CD5 gene from a rabbit cosmid library , using a probe derived from human CD5 cDNA .
	manualset3
189123	4	415476	7	NULL	NULL	0	NULL	human CD5 cDNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate this we cloned the CD5 gene from a rabbit cosmid library , using a probe derived from human CD5 cDNA .
	manualset3
189124	1	415477	7	NULL	NULL	0	NULL	video transects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate why , we used video transects and underwater photography to determine the composition , structure and status of a coral-ground community located on the edge of a rocky terrace in front of a tourist park , Xcaret , in the northern Mesoamerican Reef tract , Mexico .
	manualset3
189125	2	415477	7	NULL	NULL	0	NULL	underwater photography	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate why , we used video transects and underwater photography to determine the composition , structure and status of a coral-ground community located on the edge of a rocky terrace in front of a tourist park , Xcaret , in the northern Mesoamerican Reef tract , Mexico .
	manualset3
189126	3	415477	7	NULL	NULL	0	NULL	composition	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate why , we used video transects and underwater photography to determine the composition , structure and status of a coral-ground community located on the edge of a rocky terrace in front of a tourist park , Xcaret , in the northern Mesoamerican Reef tract , Mexico .
	manualset3
189127	4	415477	7	NULL	NULL	0	NULL	structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate why , we used video transects and underwater photography to determine the composition , structure and status of a coral-ground community located on the edge of a rocky terrace in front of a tourist park , Xcaret , in the northern Mesoamerican Reef tract , Mexico .
	manualset3
189128	5	415477	7	NULL	NULL	0	NULL	status	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate why , we used video transects and underwater photography to determine the composition , structure and status of a coral-ground community located on the edge of a rocky terrace in front of a tourist park , Xcaret , in the northern Mesoamerican Reef tract , Mexico .
	manualset3
189129	6	415477	7	NULL	NULL	0	NULL	coral-ground community	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate why , we used video transects and underwater photography to determine the composition , structure and status of a coral-ground community located on the edge of a rocky terrace in front of a tourist park , Xcaret , in the northern Mesoamerican Reef tract , Mexico .
	manualset3
189130	7	415477	7	NULL	NULL	NULL	NULL	edge of a rocky terrace 	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To investigate why , we used video transects and underwater photography to determine the composition , structure and status of a coral-ground community located on the edge of a rocky terrace in front of a tourist park , Xcaret , in the northern Mesoamerican Reef tract , Mexico .
	manualset3
189131	8	415477	7	NULL	NULL	0	NULL	tourist park	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate why , we used video transects and underwater photography to determine the composition , structure and status of a coral-ground community located on the edge of a rocky terrace in front of a tourist park , Xcaret , in the northern Mesoamerican Reef tract , Mexico .
	manualset3
189132	9	415477	7	NULL	NULL	0	NULL	Xcaret	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate why , we used video transects and underwater photography to determine the composition , structure and status of a coral-ground community located on the edge of a rocky terrace in front of a tourist park , Xcaret , in the northern Mesoamerican Reef tract , Mexico .
	manualset3
189133	10	415477	7	NULL	NULL	0	NULL	northern Mesoamerican Reef tract	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate why , we used video transects and underwater photography to determine the composition , structure and status of a coral-ground community located on the edge of a rocky terrace in front of a tourist park , Xcaret , in the northern Mesoamerican Reef tract , Mexico .
	manualset3
189134	11	415477	7	NULL	NULL	0	NULL	Mexico	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate why , we used video transects and underwater photography to determine the composition , structure and status of a coral-ground community located on the edge of a rocky terrace in front of a tourist park , Xcaret , in the northern Mesoamerican Reef tract , Mexico .
	manualset3
189135	1	415478	7	NULL	NULL	0	NULL	injection volume 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To keep the injection volume constant , each extract dose was made up 2.4 mL/Kg B.W. with olive oil .
	manualset3
189136	2	415478	7	NULL	NULL	0	NULL	extract dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To keep the injection volume constant , each extract dose was made up 2.4 mL/Kg B.W. with olive oil .
	manualset3
189137	3	415478	7	NULL	NULL	0	NULL	2.4 mL/Kg B.W.	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	To keep the injection volume constant , each extract dose was made up 2.4 mL/Kg B.W. with olive oil .
	manualset3
189138	4	415478	7	NULL	NULL	0	NULL	 olive oil	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To keep the injection volume constant , each extract dose was made up 2.4 mL/Kg B.W. with olive oil .
	manualset3
189139	1	415479	7	NULL	NULL	0	NULL	cartilage nodules 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After cartilage nodules were present , prostaglandin-E2 responsiveness decreased to about 25-fold , whereas there was no significant change in PTH responsiveness .
	manualset3
189140	2	415479	7	NULL	NULL	0	NULL	prostaglandin-E2 responsiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After cartilage nodules were present , prostaglandin-E2 responsiveness decreased to about 25-fold , whereas there was no significant change in PTH responsiveness .
	manualset3
189141	3	415479	7	NULL	NULL	0	NULL	25-fold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After cartilage nodules were present , prostaglandin-E2 responsiveness decreased to about 25-fold , whereas there was no significant change in PTH responsiveness .
	manualset3
189142	4	415479	7	NULL	NULL	0	NULL	significant change	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After cartilage nodules were present , prostaglandin-E2 responsiveness decreased to about 25-fold , whereas there was no significant change in PTH responsiveness .
	manualset3
189143	5	415479	7	NULL	NULL	0	NULL	PTH responsiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After cartilage nodules were present , prostaglandin-E2 responsiveness decreased to about 25-fold , whereas there was no significant change in PTH responsiveness .
	manualset3
189144	1	415480	7	NULL	NULL	0	NULL	IgE increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To know whether the IgE increase was related to a possible local production the AH/serum concentration ratio for IgE was calculated and divided by that for albumin .
	manualset3
189145	2	415480	7	NULL	NULL	0	NULL	local production 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To know whether the IgE increase was related to a possible local production the AH/serum concentration ratio for IgE was calculated and divided by that for albumin .
	manualset3
189146	3	415480	7	NULL	NULL	NULL	NULL	AH/serum concentration ratio	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To know whether the IgE increase was related to a possible local production the AH/serum concentration ratio for IgE was calculated and divided by that for albumin .
	manualset3
189147	4	415480	7	NULL	NULL	0	NULL	IgE	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To know whether the IgE increase was related to a possible local production the AH/serum concentration ratio for IgE was calculated and divided by that for albumin .
	manualset3
189148	5	415480	7	NULL	NULL	0	NULL	albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To know whether the IgE increase was related to a possible local production the AH/serum concentration ratio for IgE was calculated and divided by that for albumin .
	manualset3
189149	1	415481	7	NULL	NULL	0	NULL	bones 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To maintain the bones of women above the fracture threshold until the age of 70 years about 50 % of postmenopausal women need hormone replacement therapy .
	manualset3
189150	2	415481	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To maintain the bones of women above the fracture threshold until the age of 70 years about 50 % of postmenopausal women need hormone replacement therapy .
	manualset3
189151	3	415481	7	NULL	NULL	0	NULL	fracture threshold	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To maintain the bones of women above the fracture threshold until the age of 70 years about 50 % of postmenopausal women need hormone replacement therapy .
	manualset3
189152	4	415481	7	NULL	NULL	0	NULL	age	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	To maintain the bones of women above the fracture threshold until the age of 70 years about 50 % of postmenopausal women need hormone replacement therapy .
	manualset3
189153	5	415481	7	NULL	NULL	0	NULL	70 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	To maintain the bones of women above the fracture threshold until the age of 70 years about 50 % of postmenopausal women need hormone replacement therapy .
	manualset3
189154	6	415481	7	NULL	NULL	0	NULL	50 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To maintain the bones of women above the fracture threshold until the age of 70 years about 50 % of postmenopausal women need hormone replacement therapy .
	manualset3
189155	7	415481	7	NULL	NULL	0	NULL	postmenopausal women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To maintain the bones of women above the fracture threshold until the age of 70 years about 50 % of postmenopausal women need hormone replacement therapy .
	manualset3
189156	8	415481	7	NULL	NULL	0	NULL	hormone replacement therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To maintain the bones of women above the fracture threshold until the age of 70 years about 50 % of postmenopausal women need hormone replacement therapy .
	manualset3
189157	1	415482	7	NULL	NULL	0	NULL	electroneutrality	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To maintain the electroneutrality of the system , charge compensation is through oxygen vacancies which results in the brownmillerite-type structure .
	manualset3
189158	2	415482	7	NULL	NULL	0	NULL	 system	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To maintain the electroneutrality of the system , charge compensation is through oxygen vacancies which results in the brownmillerite-type structure .
	manualset3
189159	3	415482	7	NULL	NULL	0	NULL	charge compensation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To maintain the electroneutrality of the system , charge compensation is through oxygen vacancies which results in the brownmillerite-type structure .
	manualset3
189160	4	415482	7	NULL	NULL	0	NULL	oxygen vacancies	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To maintain the electroneutrality of the system , charge compensation is through oxygen vacancies which results in the brownmillerite-type structure .
	manualset3
189161	5	415482	7	NULL	NULL	0	NULL	brownmillerite-type structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To maintain the electroneutrality of the system , charge compensation is through oxygen vacancies which results in the brownmillerite-type structure .
	manualset3
189162	1	415483	7	NULL	NULL	0	NULL	cellular activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To measure cellular activation , we assessed changes in endothelial cell intracellular calcium ( ( Ca2 + ) i ) in endothelial monolayers loaded with Fura-2 , and PAF production by ( 3H ) acetate incorporation into phospholipid .
	manualset3
189163	2	415483	7	NULL	NULL	0	NULL	changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To measure cellular activation , we assessed changes in endothelial cell intracellular calcium ( ( Ca2 + ) i ) in endothelial monolayers loaded with Fura-2 , and PAF production by ( 3H ) acetate incorporation into phospholipid .
	manualset3
189164	3	415483	7	NULL	NULL	0	NULL	endothelial cell intracellular calcium ( ( Ca2 + ) i )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To measure cellular activation , we assessed changes in endothelial cell intracellular calcium ( ( Ca2 + ) i ) in endothelial monolayers loaded with Fura-2 , and PAF production by ( 3H ) acetate incorporation into phospholipid .
	manualset3
189165	4	415483	7	NULL	NULL	0	NULL	endothelial monolayers	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To measure cellular activation , we assessed changes in endothelial cell intracellular calcium ( ( Ca2 + ) i ) in endothelial monolayers loaded with Fura-2 , and PAF production by ( 3H ) acetate incorporation into phospholipid .
	manualset3
189166	5	415483	7	NULL	NULL	0	NULL	Fura-2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To measure cellular activation , we assessed changes in endothelial cell intracellular calcium ( ( Ca2 + ) i ) in endothelial monolayers loaded with Fura-2 , and PAF production by ( 3H ) acetate incorporation into phospholipid .
	manualset3
189167	6	415483	7	NULL	NULL	0	NULL	PAF production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To measure cellular activation , we assessed changes in endothelial cell intracellular calcium ( ( Ca2 + ) i ) in endothelial monolayers loaded with Fura-2 , and PAF production by ( 3H ) acetate incorporation into phospholipid .
	manualset3
189168	7	415483	7	NULL	NULL	0	NULL	( 3H ) acetate incorporation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To measure cellular activation , we assessed changes in endothelial cell intracellular calcium ( ( Ca2 + ) i ) in endothelial monolayers loaded with Fura-2 , and PAF production by ( 3H ) acetate incorporation into phospholipid .
	manualset3
189169	8	415483	7	NULL	NULL	0	NULL	phospholipid 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To measure cellular activation , we assessed changes in endothelial cell intracellular calcium ( ( Ca2 + ) i ) in endothelial monolayers loaded with Fura-2 , and PAF production by ( 3H ) acetate incorporation into phospholipid .
	manualset3
189170	1	415484	7	NULL	NULL	0	NULL	grip force distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To measure grip force distribution on a tool handle , Force Sensing Resistors were calibrated , placed on two different types of grip ( wood and foam ) and interfaced to a personal computer .
	manualset3
189171	2	415484	7	NULL	NULL	0	NULL	tool handle	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	To measure grip force distribution on a tool handle , Force Sensing Resistors were calibrated , placed on two different types of grip ( wood and foam ) and interfaced to a personal computer .
	manualset3
189172	3	415484	7	NULL	NULL	0	NULL	Force Sensing Resistors	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	To measure grip force distribution on a tool handle , Force Sensing Resistors were calibrated , placed on two different types of grip ( wood and foam ) and interfaced to a personal computer .
	manualset3
189173	4	415484	7	NULL	NULL	0	NULL	two different types	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To measure grip force distribution on a tool handle , Force Sensing Resistors were calibrated , placed on two different types of grip ( wood and foam ) and interfaced to a personal computer .
	manualset3
189174	5	415484	7	NULL	NULL	NULL	NULL	 grip	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To measure grip force distribution on a tool handle , Force Sensing Resistors were calibrated , placed on two different types of grip ( wood and foam ) and interfaced to a personal computer .
	manualset3
189175	6	415484	7	NULL	NULL	NULL	NULL	wood	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To measure grip force distribution on a tool handle , Force Sensing Resistors were calibrated , placed on two different types of grip ( wood and foam ) and interfaced to a personal computer .
	manualset3
189176	7	415484	7	NULL	NULL	NULL	NULL	foam	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To measure grip force distribution on a tool handle , Force Sensing Resistors were calibrated , placed on two different types of grip ( wood and foam ) and interfaced to a personal computer .
	manualset3
189177	8	415484	7	NULL	NULL	0	NULL	personal computer	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	To measure grip force distribution on a tool handle , Force Sensing Resistors were calibrated , placed on two different types of grip ( wood and foam ) and interfaced to a personal computer .
	manualset3
189178	1	415485	7	NULL	NULL	0	NULL	model	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To model the channel-like nature of these planes , collagen was cast in elliptical gels with major and minor axes matching the large and small circular gels , respectively , and in planar gels constrained on two sides .
	manualset3
189179	2	415485	7	NULL	NULL	0	NULL	channel-like nature	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To model the channel-like nature of these planes , collagen was cast in elliptical gels with major and minor axes matching the large and small circular gels , respectively , and in planar gels constrained on two sides .
	manualset3
189180	3	415485	7	NULL	NULL	0	NULL	planes 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To model the channel-like nature of these planes , collagen was cast in elliptical gels with major and minor axes matching the large and small circular gels , respectively , and in planar gels constrained on two sides .
	manualset3
189181	4	415485	7	NULL	NULL	0	NULL	collagen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To model the channel-like nature of these planes , collagen was cast in elliptical gels with major and minor axes matching the large and small circular gels , respectively , and in planar gels constrained on two sides .
	manualset3
189182	5	415485	7	NULL	NULL	NULL	NULL	elliptical gels	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To model the channel-like nature of these planes , collagen was cast in elliptical gels with major and minor axes matching the large and small circular gels , respectively , and in planar gels constrained on two sides .
	manualset3
189183	6	415485	7	NULL	NULL	NULL	NULL	major axes	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To model the channel-like nature of these planes , collagen was cast in elliptical gels with major and minor axes matching the large and small circular gels , respectively , and in planar gels constrained on two sides .
	manualset3
189184	7	415485	7	NULL	NULL	NULL	NULL	minor axes	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To model the channel-like nature of these planes , collagen was cast in elliptical gels with major and minor axes matching the large and small circular gels , respectively , and in planar gels constrained on two sides .
	manualset3
189185	8	415485	7	NULL	NULL	0	NULL	 large gels	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To model the channel-like nature of these planes , collagen was cast in elliptical gels with major and minor axes matching the large and small circular gels , respectively , and in planar gels constrained on two sides .
	manualset3
189186	9	415485	7	NULL	NULL	0	NULL	small circular gels	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To model the channel-like nature of these planes , collagen was cast in elliptical gels with major and minor axes matching the large and small circular gels , respectively , and in planar gels constrained on two sides .
	manualset3
189187	10	415485	7	NULL	NULL	0	NULL	planar gels 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To model the channel-like nature of these planes , collagen was cast in elliptical gels with major and minor axes matching the large and small circular gels , respectively , and in planar gels constrained on two sides .
	manualset3
189188	11	415485	7	NULL	NULL	0	NULL	two sides	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	To model the channel-like nature of these planes , collagen was cast in elliptical gels with major and minor axes matching the large and small circular gels , respectively , and in planar gels constrained on two sides .
	manualset3
189189	1	415486	7	NULL	NULL	0	NULL	 heartrate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To obtain an accurate heartrate , the ECG signals have to be analyzed and calculations performed to find occurrences of the QRS complex , a major component of the ECG signal .
	manualset3
189190	2	415486	7	NULL	NULL	0	NULL	ECG signals	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To obtain an accurate heartrate , the ECG signals have to be analyzed and calculations performed to find occurrences of the QRS complex , a major component of the ECG signal .
	manualset3
189191	3	415486	7	NULL	NULL	0	NULL	calculations	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	To obtain an accurate heartrate , the ECG signals have to be analyzed and calculations performed to find occurrences of the QRS complex , a major component of the ECG signal .
	manualset3
189192	4	415486	7	NULL	NULL	0	NULL	QRS complex	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To obtain an accurate heartrate , the ECG signals have to be analyzed and calculations performed to find occurrences of the QRS complex , a major component of the ECG signal .
	manualset3
189193	5	415486	7	NULL	NULL	0	NULL	major component	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To obtain an accurate heartrate , the ECG signals have to be analyzed and calculations performed to find occurrences of the QRS complex , a major component of the ECG signal .
	manualset3
189194	6	415486	7	NULL	NULL	0	NULL	ECG signal	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To obtain an accurate heartrate , the ECG signals have to be analyzed and calculations performed to find occurrences of the QRS complex , a major component of the ECG signal .
	manualset3
191683	7	415486	7	NULL	NULL	0	NULL	occurrences	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To obtain an accurate heartrate , the ECG signals have to be analyzed and calculations performed to find occurrences of the QRS complex , a major component of the ECG signal .
	manualset3
189195	1	415487	7	NULL	NULL	0	NULL	 information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	To obtain information to guide future health care planning , data from government and other sources on the demographic and medical characteristics of menopausal Taiwanese women were reviewed .
	manualset3
189196	2	415487	7	NULL	NULL	0	NULL	health care planning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To obtain information to guide future health care planning , data from government and other sources on the demographic and medical characteristics of menopausal Taiwanese women were reviewed .
	manualset3
189197	3	415487	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	To obtain information to guide future health care planning , data from government and other sources on the demographic and medical characteristics of menopausal Taiwanese women were reviewed .
	manualset3
189198	4	415487	7	NULL	NULL	0	NULL	government	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	To obtain information to guide future health care planning , data from government and other sources on the demographic and medical characteristics of menopausal Taiwanese women were reviewed .
	manualset3
189199	5	415487	7	NULL	NULL	0	NULL	sources	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To obtain information to guide future health care planning , data from government and other sources on the demographic and medical characteristics of menopausal Taiwanese women were reviewed .
	manualset3
189200	6	415487	7	NULL	NULL	0	NULL	demographic characteristics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To obtain information to guide future health care planning , data from government and other sources on the demographic and medical characteristics of menopausal Taiwanese women were reviewed .
	manualset3
189201	7	415487	7	NULL	NULL	0	NULL	medical characteristics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To obtain information to guide future health care planning , data from government and other sources on the demographic and medical characteristics of menopausal Taiwanese women were reviewed .
	manualset3
189202	8	415487	7	NULL	NULL	0	NULL	menopausal Taiwanese women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To obtain information to guide future health care planning , data from government and other sources on the demographic and medical characteristics of menopausal Taiwanese women were reviewed .
	manualset3
189203	1	415488	7	NULL	NULL	0	NULL	two-dimensional ( 2D ) THz images	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	To obtain the two-dimensional ( 2D ) THz images of samples , the laser pulses are scanned over a 2D THz emitter plate ( DASC : 4 ' - dimenthylamino-N-methyl-4 - stilbazolium p-chlorobenzenesulfonate ) by a galvano meter .
	manualset3
189204	2	415488	7	NULL	NULL	0	NULL	samples	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To obtain the two-dimensional ( 2D ) THz images of samples , the laser pulses are scanned over a 2D THz emitter plate ( DASC : 4 ' - dimenthylamino-N-methyl-4 - stilbazolium p-chlorobenzenesulfonate ) by a galvano meter .
	manualset3
189205	3	415488	7	NULL	NULL	0	NULL	laser pulses	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	To obtain the two-dimensional ( 2D ) THz images of samples , the laser pulses are scanned over a 2D THz emitter plate ( DASC : 4 ' - dimenthylamino-N-methyl-4 - stilbazolium p-chlorobenzenesulfonate ) by a galvano meter .
	manualset3
189206	4	415488	7	NULL	NULL	0	NULL	2D THz emitter plate	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	To obtain the two-dimensional ( 2D ) THz images of samples , the laser pulses are scanned over a 2D THz emitter plate ( DASC : 4 ' - dimenthylamino-N-methyl-4 - stilbazolium p-chlorobenzenesulfonate ) by a galvano meter .
	manualset3
189207	5	415488	7	NULL	NULL	0	NULL	DASC : 4 ' - dimenthylamino-N-methyl-4 - stilbazolium p-chlorobenzenesulfonate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To obtain the two-dimensional ( 2D ) THz images of samples , the laser pulses are scanned over a 2D THz emitter plate ( DASC : 4 ' - dimenthylamino-N-methyl-4 - stilbazolium p-chlorobenzenesulfonate ) by a galvano meter .
	manualset3
189208	6	415488	7	NULL	NULL	0	NULL	galvano meter	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	To obtain the two-dimensional ( 2D ) THz images of samples , the laser pulses are scanned over a 2D THz emitter plate ( DASC : 4 ' - dimenthylamino-N-methyl-4 - stilbazolium p-chlorobenzenesulfonate ) by a galvano meter .
	manualset3
189209	1	415489	7	NULL	NULL	0	NULL	BTV 17	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	After challenge with BTV 17 the sheep in both groups remained clinically normal , and virus was not detected in the blood ; however , serum neutralizing antibody titers to both viruses increased 2 weeks after challenge and the mean titer of the two groups ranged from 1 : 250 to 1 : 640 .
	manualset3
189210	2	415489	7	NULL	NULL	0	NULL	sheep	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	After challenge with BTV 17 the sheep in both groups remained clinically normal , and virus was not detected in the blood ; however , serum neutralizing antibody titers to both viruses increased 2 weeks after challenge and the mean titer of the two groups ranged from 1 : 250 to 1 : 640 .
	manualset3
189211	3	415489	7	NULL	NULL	0	NULL	groups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	After challenge with BTV 17 the sheep in both groups remained clinically normal , and virus was not detected in the blood ; however , serum neutralizing antibody titers to both viruses increased 2 weeks after challenge and the mean titer of the two groups ranged from 1 : 250 to 1 : 640 .
	manualset3
189212	4	415489	7	NULL	NULL	0	NULL	 virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	After challenge with BTV 17 the sheep in both groups remained clinically normal , and virus was not detected in the blood ; however , serum neutralizing antibody titers to both viruses increased 2 weeks after challenge and the mean titer of the two groups ranged from 1 : 250 to 1 : 640 .
	manualset3
189213	5	415489	7	NULL	NULL	0	NULL	blood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After challenge with BTV 17 the sheep in both groups remained clinically normal , and virus was not detected in the blood ; however , serum neutralizing antibody titers to both viruses increased 2 weeks after challenge and the mean titer of the two groups ranged from 1 : 250 to 1 : 640 .
	manualset3
189214	6	415489	7	NULL	NULL	0	NULL	serum neutralizing antibody titers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After challenge with BTV 17 the sheep in both groups remained clinically normal , and virus was not detected in the blood ; however , serum neutralizing antibody titers to both viruses increased 2 weeks after challenge and the mean titer of the two groups ranged from 1 : 250 to 1 : 640 .
	manualset3
189215	7	415489	7	NULL	NULL	0	NULL	viruses 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	After challenge with BTV 17 the sheep in both groups remained clinically normal , and virus was not detected in the blood ; however , serum neutralizing antibody titers to both viruses increased 2 weeks after challenge and the mean titer of the two groups ranged from 1 : 250 to 1 : 640 .
	manualset3
189216	8	415489	7	NULL	NULL	0	NULL	2 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After challenge with BTV 17 the sheep in both groups remained clinically normal , and virus was not detected in the blood ; however , serum neutralizing antibody titers to both viruses increased 2 weeks after challenge and the mean titer of the two groups ranged from 1 : 250 to 1 : 640 .
	manualset3
189217	9	415489	7	NULL	NULL	0	NULL	mean titer	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After challenge with BTV 17 the sheep in both groups remained clinically normal , and virus was not detected in the blood ; however , serum neutralizing antibody titers to both viruses increased 2 weeks after challenge and the mean titer of the two groups ranged from 1 : 250 to 1 : 640 .
	manualset3
189218	10	415489	7	NULL	NULL	0	NULL	two groups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	After challenge with BTV 17 the sheep in both groups remained clinically normal , and virus was not detected in the blood ; however , serum neutralizing antibody titers to both viruses increased 2 weeks after challenge and the mean titer of the two groups ranged from 1 : 250 to 1 : 640 .
	manualset3
189219	11	415489	7	NULL	NULL	0	NULL	1 : 250	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	After challenge with BTV 17 the sheep in both groups remained clinically normal , and virus was not detected in the blood ; however , serum neutralizing antibody titers to both viruses increased 2 weeks after challenge and the mean titer of the two groups ranged from 1 : 250 to 1 : 640 .
	manualset3
189220	12	415489	7	NULL	NULL	0	NULL	1 : 640	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	After challenge with BTV 17 the sheep in both groups remained clinically normal , and virus was not detected in the blood ; however , serum neutralizing antibody titers to both viruses increased 2 weeks after challenge and the mean titer of the two groups ranged from 1 : 250 to 1 : 640 .
	manualset3
189221	1	415490	7	NULL	NULL	0	NULL	R479	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , R479 is the first porcine-bovine reassortant rotavirus isolated from a human .
	manualset3
189222	2	415490	7	NULL	NULL	0	NULL	porcine-bovine reassortant rotavirus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , R479 is the first porcine-bovine reassortant rotavirus isolated from a human .
	manualset3
189223	3	415490	7	NULL	NULL	0	NULL	human	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , R479 is the first porcine-bovine reassortant rotavirus isolated from a human .
	manualset3
189224	4	415490	7	NULL	NULL	0	NULL	knowledge	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , R479 is the first porcine-bovine reassortant rotavirus isolated from a human .
	manualset3
189225	1	415491	7	NULL	NULL	0	NULL	knowledge	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , the 50-kDa subunit is the first example of a functional beta-subunit-like protein in vertebrates .
	manualset3
189226	2	415491	7	NULL	NULL	0	NULL	50-kDa subunit	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , the 50-kDa subunit is the first example of a functional beta-subunit-like protein in vertebrates .
	manualset3
189227	3	415491	7	NULL	NULL	0	NULL	 example	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , the 50-kDa subunit is the first example of a functional beta-subunit-like protein in vertebrates .
	manualset3
189228	4	415491	7	NULL	NULL	0	NULL	 functional beta-subunit-like protein	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , the 50-kDa subunit is the first example of a functional beta-subunit-like protein in vertebrates .
	manualset3
189229	5	415491	7	NULL	NULL	0	NULL	vertebrates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , the 50-kDa subunit is the first example of a functional beta-subunit-like protein in vertebrates .
	manualset3
189230	1	415492	7	NULL	NULL	0	NULL	knowledge	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this balanced translocation , namely t ( 3 ; 14 ) ( p21 .1 ; q24 .1 ) , which is present both in the patient with MDS with erythroid hypoplasia and in the healthy members of the family , has not been defined previously .
	manualset3
189231	2	415492	7	NULL	NULL	0	NULL	balanced translocation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this balanced translocation , namely t ( 3 ; 14 ) ( p21 .1 ; q24 .1 ) , which is present both in the patient with MDS with erythroid hypoplasia and in the healthy members of the family , has not been defined previously .
	manualset3
189232	3	415492	7	NULL	NULL	0	NULL	t ( 3 ; 14 ) ( p21 .1 ; q24 .1 ) 	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this balanced translocation , namely t ( 3 ; 14 ) ( p21 .1 ; q24 .1 ) , which is present both in the patient with MDS with erythroid hypoplasia and in the healthy members of the family , has not been defined previously .
	manualset3
189233	4	415492	7	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this balanced translocation , namely t ( 3 ; 14 ) ( p21 .1 ; q24 .1 ) , which is present both in the patient with MDS with erythroid hypoplasia and in the healthy members of the family , has not been defined previously .
	manualset3
189234	5	415492	7	NULL	NULL	0	NULL	MDS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this balanced translocation , namely t ( 3 ; 14 ) ( p21 .1 ; q24 .1 ) , which is present both in the patient with MDS with erythroid hypoplasia and in the healthy members of the family , has not been defined previously .
	manualset3
189235	6	415492	7	NULL	NULL	0	NULL	erythroid hypoplasia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this balanced translocation , namely t ( 3 ; 14 ) ( p21 .1 ; q24 .1 ) , which is present both in the patient with MDS with erythroid hypoplasia and in the healthy members of the family , has not been defined previously .
	manualset3
189236	7	415492	7	NULL	NULL	0	NULL	healthy members 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this balanced translocation , namely t ( 3 ; 14 ) ( p21 .1 ; q24 .1 ) , which is present both in the patient with MDS with erythroid hypoplasia and in the healthy members of the family , has not been defined previously .
	manualset3
189237	8	415492	7	NULL	NULL	0	NULL	family	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this balanced translocation , namely t ( 3 ; 14 ) ( p21 .1 ; q24 .1 ) , which is present both in the patient with MDS with erythroid hypoplasia and in the healthy members of the family , has not been defined previously .
	manualset3
189238	1	415493	7	NULL	NULL	0	NULL	knowledge	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this is the first report showing the possible association of Cdt-producing E. coli in Japan , particularly in a child with bloody diarrhea .
	manualset3
189239	2	415493	7	NULL	NULL	0	NULL	first report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this is the first report showing the possible association of Cdt-producing E. coli in Japan , particularly in a child with bloody diarrhea .
	manualset3
189240	3	415493	7	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this is the first report showing the possible association of Cdt-producing E. coli in Japan , particularly in a child with bloody diarrhea .
	manualset3
189241	4	415493	7	NULL	NULL	0	NULL	Cdt-producing E. coli 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this is the first report showing the possible association of Cdt-producing E. coli in Japan , particularly in a child with bloody diarrhea .
	manualset3
189242	5	415493	7	NULL	NULL	0	NULL	Japan	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this is the first report showing the possible association of Cdt-producing E. coli in Japan , particularly in a child with bloody diarrhea .
	manualset3
189243	6	415493	7	NULL	NULL	0	NULL	child	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this is the first report showing the possible association of Cdt-producing E. coli in Japan , particularly in a child with bloody diarrhea .
	manualset3
189244	7	415493	7	NULL	NULL	NULL	NULL	bloody diarrhea	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To our knowledge , this is the first report showing the possible association of Cdt-producing E. coli in Japan , particularly in a child with bloody diarrhea .
	manualset3
189245	1	415494	7	NULL	NULL	0	NULL	knowledge	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this is the first reported case on the species L. xyli exhibited R-stereospecific carbonyl reductase and used for the preparation of chiral ( 1R ) - ( 3 , 5-bis ( trifluoromethyl ) phenyl ) ethanol .
	manualset3
189246	2	415494	7	NULL	NULL	0	NULL	first reported case	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this is the first reported case on the species L. xyli exhibited R-stereospecific carbonyl reductase and used for the preparation of chiral ( 1R ) - ( 3 , 5-bis ( trifluoromethyl ) phenyl ) ethanol .
	manualset3
189247	3	415494	7	NULL	NULL	0	NULL	species L. xyli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this is the first reported case on the species L. xyli exhibited R-stereospecific carbonyl reductase and used for the preparation of chiral ( 1R ) - ( 3 , 5-bis ( trifluoromethyl ) phenyl ) ethanol .
	manualset3
189248	4	415494	7	NULL	NULL	0	NULL	R-stereospecific carbonyl reductase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this is the first reported case on the species L. xyli exhibited R-stereospecific carbonyl reductase and used for the preparation of chiral ( 1R ) - ( 3 , 5-bis ( trifluoromethyl ) phenyl ) ethanol .
	manualset3
189249	5	415494	7	NULL	NULL	0	NULL	 preparation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this is the first reported case on the species L. xyli exhibited R-stereospecific carbonyl reductase and used for the preparation of chiral ( 1R ) - ( 3 , 5-bis ( trifluoromethyl ) phenyl ) ethanol .
	manualset3
189250	6	415494	7	NULL	NULL	0	NULL	chiral ( 1R ) - ( 3 , 5-bis ( trifluoromethyl ) phenyl ) ethanol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this is the first reported case on the species L. xyli exhibited R-stereospecific carbonyl reductase and used for the preparation of chiral ( 1R ) - ( 3 , 5-bis ( trifluoromethyl ) phenyl ) ethanol .
	manualset3
189251	1	415495	7	NULL	NULL	0	NULL	knowledge	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this is the second report of laparoscopic diagnosis and treatment of an epipolic disorder .
	manualset3
189252	2	415495	7	NULL	NULL	0	NULL	second report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this is the second report of laparoscopic diagnosis and treatment of an epipolic disorder .
	manualset3
189253	3	415495	7	NULL	NULL	0	NULL	laparoscopic diagnosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this is the second report of laparoscopic diagnosis and treatment of an epipolic disorder .
	manualset3
189254	4	415495	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this is the second report of laparoscopic diagnosis and treatment of an epipolic disorder .
	manualset3
189255	5	415495	7	NULL	NULL	0	NULL	epipolic disorder	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this is the second report of laparoscopic diagnosis and treatment of an epipolic disorder .
	manualset3
189256	1	415496	7	NULL	NULL	0	NULL	knowledge	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this study is the first example of detection of a mutation in the RBD-I of PKR gene from tumor cells taken directly from patients .
	manualset3
189257	2	415496	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this study is the first example of detection of a mutation in the RBD-I of PKR gene from tumor cells taken directly from patients .
	manualset3
189258	3	415496	7	NULL	NULL	0	NULL	example 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this study is the first example of detection of a mutation in the RBD-I of PKR gene from tumor cells taken directly from patients .
	manualset3
189259	4	415496	7	NULL	NULL	0	NULL	detection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this study is the first example of detection of a mutation in the RBD-I of PKR gene from tumor cells taken directly from patients .
	manualset3
189260	5	415496	7	NULL	NULL	0	NULL	 mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this study is the first example of detection of a mutation in the RBD-I of PKR gene from tumor cells taken directly from patients .
	manualset3
189261	6	415496	7	NULL	NULL	0	NULL	 RBD-I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this study is the first example of detection of a mutation in the RBD-I of PKR gene from tumor cells taken directly from patients .
	manualset3
189262	7	415496	7	NULL	NULL	0	NULL	PKR gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this study is the first example of detection of a mutation in the RBD-I of PKR gene from tumor cells taken directly from patients .
	manualset3
189263	8	415496	7	NULL	NULL	0	NULL	tumor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this study is the first example of detection of a mutation in the RBD-I of PKR gene from tumor cells taken directly from patients .
	manualset3
189264	9	415496	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To our knowledge , this study is the first example of detection of a mutation in the RBD-I of PKR gene from tumor cells taken directly from patients .
	manualset3
189265	1	415497	7	NULL	NULL	0	NULL	Concentration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Concentration of C1-esterase-inhibitor in coagulation-active plasma samples ) .
	manualset3
189266	2	415497	7	NULL	NULL	0	NULL	C1-esterase-inhibitor	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Concentration of C1-esterase-inhibitor in coagulation-active plasma samples ) .
	manualset3
189267	3	415497	7	NULL	NULL	NULL	NULL	coagulation-active plasma samples 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Concentration of C1-esterase-inhibitor in coagulation-active plasma samples ) .
	manualset3
189268	1	415498	7	NULL	NULL	0	NULL	 chronic exposure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After chronic exposure FOC significantly delayed the first day of reproduction and decreased the number of young and growth rate even at 10 ng/l FOC .
	manualset3
189269	2	415498	7	NULL	NULL	0	NULL	FOC	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After chronic exposure FOC significantly delayed the first day of reproduction and decreased the number of young and growth rate even at 10 ng/l FOC .
	manualset3
189270	3	415498	7	NULL	NULL	0	NULL	first day	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After chronic exposure FOC significantly delayed the first day of reproduction and decreased the number of young and growth rate even at 10 ng/l FOC .
	manualset3
189271	4	415498	7	NULL	NULL	0	NULL	reproduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After chronic exposure FOC significantly delayed the first day of reproduction and decreased the number of young and growth rate even at 10 ng/l FOC .
	manualset3
189272	5	415498	7	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After chronic exposure FOC significantly delayed the first day of reproduction and decreased the number of young and growth rate even at 10 ng/l FOC .
	manualset3
189273	6	415498	7	NULL	NULL	0	NULL	 young	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	After chronic exposure FOC significantly delayed the first day of reproduction and decreased the number of young and growth rate even at 10 ng/l FOC .
	manualset3
189274	7	415498	7	NULL	NULL	0	NULL	growth rate 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After chronic exposure FOC significantly delayed the first day of reproduction and decreased the number of young and growth rate even at 10 ng/l FOC .
	manualset3
189275	8	415498	7	NULL	NULL	0	NULL	10 ng/l FOC	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	After chronic exposure FOC significantly delayed the first day of reproduction and decreased the number of young and growth rate even at 10 ng/l FOC .
	manualset3
189276	1	415499	7	NULL	NULL	0	NULL	nurses	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To practice effectively , nurses must readjust their roles and training .
	manualset3
189277	2	415499	7	NULL	NULL	0	NULL	roles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To practice effectively , nurses must readjust their roles and training .
	manualset3
189278	3	415499	7	NULL	NULL	0	NULL	training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To practice effectively , nurses must readjust their roles and training .
	manualset3
189279	1	415500	7	NULL	NULL	0	NULL	 heat-labile , short-lived `` danger signals	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To preserve heat-labile , short-lived `` danger signals , '' we induced necrosis by mechanical stress .
	manualset3
189280	2	415500	7	NULL	NULL	0	NULL	necrosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To preserve heat-labile , short-lived `` danger signals , '' we induced necrosis by mechanical stress .
	manualset3
189281	3	415500	7	NULL	NULL	0	NULL	mechanical stress	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	To preserve heat-labile , short-lived `` danger signals , '' we induced necrosis by mechanical stress .
	manualset3
189282	1	415501	7	NULL	NULL	NULL	NULL	 potentially life-threatening pressure ulcers	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To prevent disfiguring and potentially life-threatening pressure ulcers , it is important that risk factors are identified and minimized .
	manualset3
189283	2	415501	7	NULL	NULL	0	NULL	risk factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To prevent disfiguring and potentially life-threatening pressure ulcers , it is important that risk factors are identified and minimized .
	manualset3
189284	1	415502	7	NULL	NULL	0	NULL	instability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To prevent this instability , we performed a stabilization technique using an anconeus muscle flap .
	manualset3
189285	2	415502	7	NULL	NULL	0	NULL	stabilization technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To prevent this instability , we performed a stabilization technique using an anconeus muscle flap .
	manualset3
189286	3	415502	7	NULL	NULL	0	NULL	anconeus muscle flap	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To prevent this instability , we performed a stabilization technique using an anconeus muscle flap .
	manualset3
189287	1	415503	7	NULL	NULL	0	NULL	human macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To probe whether human macrophages express potentially functional alternative entry pathways , we analyzed cell-cell fusion and infection of primary macrophage by several SIVmac Envs .
	manualset3
189288	2	415503	7	NULL	NULL	0	NULL	alternative entry pathways 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To probe whether human macrophages express potentially functional alternative entry pathways , we analyzed cell-cell fusion and infection of primary macrophage by several SIVmac Envs .
	manualset3
189289	3	415503	7	NULL	NULL	0	NULL	cell-cell fusion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To probe whether human macrophages express potentially functional alternative entry pathways , we analyzed cell-cell fusion and infection of primary macrophage by several SIVmac Envs .
	manualset3
189290	4	415503	7	NULL	NULL	0	NULL	infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To probe whether human macrophages express potentially functional alternative entry pathways , we analyzed cell-cell fusion and infection of primary macrophage by several SIVmac Envs .
	manualset3
189291	5	415503	7	NULL	NULL	0	NULL	primary macrophage	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To probe whether human macrophages express potentially functional alternative entry pathways , we analyzed cell-cell fusion and infection of primary macrophage by several SIVmac Envs .
	manualset3
189292	6	415503	7	NULL	NULL	0	NULL	SIVmac Envs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To probe whether human macrophages express potentially functional alternative entry pathways , we analyzed cell-cell fusion and infection of primary macrophage by several SIVmac Envs .
	manualset3
189293	1	415504	7	NULL	NULL	0	NULL	bacterial invasion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To protect this bacterial invasion , murine monoclonal antibody ( MAb ) Pg-vc , which inhibited the hemagglutinating activity , was prepared by using P. gingivalis vesicles as an antigen .
	manualset3
189294	2	415504	7	NULL	NULL	0	NULL	murine monoclonal antibody ( MAb ) Pg-vc	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To protect this bacterial invasion , murine monoclonal antibody ( MAb ) Pg-vc , which inhibited the hemagglutinating activity , was prepared by using P. gingivalis vesicles as an antigen .
	manualset3
189295	3	415504	7	NULL	NULL	0	NULL	hemagglutinating activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To protect this bacterial invasion , murine monoclonal antibody ( MAb ) Pg-vc , which inhibited the hemagglutinating activity , was prepared by using P. gingivalis vesicles as an antigen .
	manualset3
189296	4	415504	7	NULL	NULL	NULL	NULL	P. gingivalis vesicles	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To protect this bacterial invasion , murine monoclonal antibody ( MAb ) Pg-vc , which inhibited the hemagglutinating activity , was prepared by using P. gingivalis vesicles as an antigen .
	manualset3
189297	5	415504	7	NULL	NULL	0	NULL	antigen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To protect this bacterial invasion , murine monoclonal antibody ( MAb ) Pg-vc , which inhibited the hemagglutinating activity , was prepared by using P. gingivalis vesicles as an antigen .
	manualset3
189298	1	415505	7	NULL	NULL	0	NULL	scientific basis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To provide a scientific basis for peptide therapy , an increasing number of CTL-directed peptides have been identified , and some of them have been tried as antigen-specific immunotherapy in the past decade .
	manualset3
189299	2	415505	7	NULL	NULL	0	NULL	peptide therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To provide a scientific basis for peptide therapy , an increasing number of CTL-directed peptides have been identified , and some of them have been tried as antigen-specific immunotherapy in the past decade .
	manualset3
189300	3	415505	7	NULL	NULL	0	NULL	increasing number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To provide a scientific basis for peptide therapy , an increasing number of CTL-directed peptides have been identified , and some of them have been tried as antigen-specific immunotherapy in the past decade .
	manualset3
189301	4	415505	7	NULL	NULL	0	NULL	CTL-directed peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	To provide a scientific basis for peptide therapy , an increasing number of CTL-directed peptides have been identified , and some of them have been tried as antigen-specific immunotherapy in the past decade .
	manualset3
189302	5	415505	7	NULL	NULL	0	NULL	antigen-specific immunotherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To provide a scientific basis for peptide therapy , an increasing number of CTL-directed peptides have been identified , and some of them have been tried as antigen-specific immunotherapy in the past decade .
	manualset3
189303	6	415505	7	NULL	NULL	0	NULL	decade	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	To provide a scientific basis for peptide therapy , an increasing number of CTL-directed peptides have been identified , and some of them have been tried as antigen-specific immunotherapy in the past decade .
	manualset3
189304	1	415506	7	NULL	NULL	0	NULL	novel insights	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To provide novel insights into the functions of DISC1 in brain development , we mapped the expression of zebrafish disc1 and set out to characterize its role in early embryonic development using morpholino antisense methods .
	manualset3
189305	2	415506	7	NULL	NULL	0	NULL	functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To provide novel insights into the functions of DISC1 in brain development , we mapped the expression of zebrafish disc1 and set out to characterize its role in early embryonic development using morpholino antisense methods .
	manualset3
189306	3	415506	7	NULL	NULL	0	NULL	DISC1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To provide novel insights into the functions of DISC1 in brain development , we mapped the expression of zebrafish disc1 and set out to characterize its role in early embryonic development using morpholino antisense methods .
	manualset3
189307	4	415506	7	NULL	NULL	0	NULL	brain development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To provide novel insights into the functions of DISC1 in brain development , we mapped the expression of zebrafish disc1 and set out to characterize its role in early embryonic development using morpholino antisense methods .
	manualset3
189308	5	415506	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To provide novel insights into the functions of DISC1 in brain development , we mapped the expression of zebrafish disc1 and set out to characterize its role in early embryonic development using morpholino antisense methods .
	manualset3
189309	6	415506	7	NULL	NULL	0	NULL	zebrafish disc1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To provide novel insights into the functions of DISC1 in brain development , we mapped the expression of zebrafish disc1 and set out to characterize its role in early embryonic development using morpholino antisense methods .
	manualset3
189310	7	415506	7	NULL	NULL	0	NULL	 role 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To provide novel insights into the functions of DISC1 in brain development , we mapped the expression of zebrafish disc1 and set out to characterize its role in early embryonic development using morpholino antisense methods .
	manualset3
189311	8	415506	7	NULL	NULL	0	NULL	 early embryonic development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To provide novel insights into the functions of DISC1 in brain development , we mapped the expression of zebrafish disc1 and set out to characterize its role in early embryonic development using morpholino antisense methods .
	manualset3
189312	9	415506	7	NULL	NULL	0	NULL	morpholino antisense methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To provide novel insights into the functions of DISC1 in brain development , we mapped the expression of zebrafish disc1 and set out to characterize its role in early embryonic development using morpholino antisense methods .
	manualset3
189313	1	415507	7	NULL	NULL	0	NULL	 control measures	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After control measures had interrupted the outbreak , a prospective microbiologic investigation demonstrated that one third of the hospital personnel had transient hand colonization with multiple strains of A. calcoaceticus .
	manualset3
189314	2	415507	7	NULL	NULL	0	NULL	outbreak	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After control measures had interrupted the outbreak , a prospective microbiologic investigation demonstrated that one third of the hospital personnel had transient hand colonization with multiple strains of A. calcoaceticus .
	manualset3
189315	3	415507	7	NULL	NULL	0	NULL	microbiologic investigation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After control measures had interrupted the outbreak , a prospective microbiologic investigation demonstrated that one third of the hospital personnel had transient hand colonization with multiple strains of A. calcoaceticus .
	manualset3
189316	4	415507	7	NULL	NULL	0	NULL	one third 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After control measures had interrupted the outbreak , a prospective microbiologic investigation demonstrated that one third of the hospital personnel had transient hand colonization with multiple strains of A. calcoaceticus .
	manualset3
189317	5	415507	7	NULL	NULL	0	NULL	hospital personnel 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	After control measures had interrupted the outbreak , a prospective microbiologic investigation demonstrated that one third of the hospital personnel had transient hand colonization with multiple strains of A. calcoaceticus .
	manualset3
189318	6	415507	7	NULL	NULL	0	NULL	transient hand colonization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After control measures had interrupted the outbreak , a prospective microbiologic investigation demonstrated that one third of the hospital personnel had transient hand colonization with multiple strains of A. calcoaceticus .
	manualset3
189319	7	415507	7	NULL	NULL	0	NULL	multiple strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	After control measures had interrupted the outbreak , a prospective microbiologic investigation demonstrated that one third of the hospital personnel had transient hand colonization with multiple strains of A. calcoaceticus .
	manualset3
189320	8	415507	7	NULL	NULL	0	NULL	A. calcoaceticus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	After control measures had interrupted the outbreak , a prospective microbiologic investigation demonstrated that one third of the hospital personnel had transient hand colonization with multiple strains of A. calcoaceticus .
	manualset3
189321	1	415508	7	NULL	NULL	0	NULL	rate of insulin absorption	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To quantify better the rate and extent of insulin absorption from the small intestine , closed-loop in situ experiments were performed in nondiabetic rats .
	manualset3
189322	2	415508	7	NULL	NULL	0	NULL	extent of insulin absorption	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To quantify better the rate and extent of insulin absorption from the small intestine , closed-loop in situ experiments were performed in nondiabetic rats .
	manualset3
189323	3	415508	7	NULL	NULL	0	NULL	small intestine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To quantify better the rate and extent of insulin absorption from the small intestine , closed-loop in situ experiments were performed in nondiabetic rats .
	manualset3
189324	4	415508	7	NULL	NULL	0	NULL	closed-loop in situ experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To quantify better the rate and extent of insulin absorption from the small intestine , closed-loop in situ experiments were performed in nondiabetic rats .
	manualset3
189325	5	415508	7	NULL	NULL	0	NULL	nondiabetic rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To quantify better the rate and extent of insulin absorption from the small intestine , closed-loop in situ experiments were performed in nondiabetic rats .
	manualset3
189326	1	415509	7	NULL	NULL	0	NULL	biological activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To quantify the biological activity of different cytokine preparations with different specific activities by bioassay , mass units can not be used and biological activity has to be expressed as & lt ; & lt ; biological potency units ) ) .
	manualset3
189327	2	415509	7	NULL	NULL	NULL	NULL	 cytokine preparations	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To quantify the biological activity of different cytokine preparations with different specific activities by bioassay , mass units can not be used and biological activity has to be expressed as & lt ; & lt ; biological potency units ) ) .
	manualset3
189328	3	415509	7	NULL	NULL	0	NULL	different specific activities	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To quantify the biological activity of different cytokine preparations with different specific activities by bioassay , mass units can not be used and biological activity has to be expressed as & lt ; & lt ; biological potency units ) ) .
	manualset3
189329	4	415509	7	NULL	NULL	0	NULL	bioassay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To quantify the biological activity of different cytokine preparations with different specific activities by bioassay , mass units can not be used and biological activity has to be expressed as & lt ; & lt ; biological potency units ) ) .
	manualset3
189330	5	415509	7	NULL	NULL	0	NULL	mass units	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To quantify the biological activity of different cytokine preparations with different specific activities by bioassay , mass units can not be used and biological activity has to be expressed as & lt ; & lt ; biological potency units ) ) .
	manualset3
189331	6	415509	7	NULL	NULL	0	NULL	biological activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To quantify the biological activity of different cytokine preparations with different specific activities by bioassay , mass units can not be used and biological activity has to be expressed as & lt ; & lt ; biological potency units ) ) .
	manualset3
189332	7	415509	7	NULL	NULL	0	NULL	& lt ; & lt 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To quantify the biological activity of different cytokine preparations with different specific activities by bioassay , mass units can not be used and biological activity has to be expressed as & lt ; & lt ; biological potency units ) ) .
	manualset3
189333	8	415509	7	NULL	NULL	0	NULL	biological potency units	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To quantify the biological activity of different cytokine preparations with different specific activities by bioassay , mass units can not be used and biological activity has to be expressed as & lt ; & lt ; biological potency units ) ) .
	manualset3
189334	1	415510	7	NULL	NULL	0	NULL	impairment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To quantify the impairment in the HRQOL , the 36-item version of the inflammatory bowel disease questionnaire ( IBDQ ) was administered to all patients .
	manualset3
189335	2	415510	7	NULL	NULL	0	NULL	HRQOL	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To quantify the impairment in the HRQOL , the 36-item version of the inflammatory bowel disease questionnaire ( IBDQ ) was administered to all patients .
	manualset3
189336	3	415510	7	NULL	NULL	0	NULL	 36-item version	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	To quantify the impairment in the HRQOL , the 36-item version of the inflammatory bowel disease questionnaire ( IBDQ ) was administered to all patients .
	manualset3
189337	4	415510	7	NULL	NULL	0	NULL	inflammatory bowel disease questionnaire ( IBDQ )	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	To quantify the impairment in the HRQOL , the 36-item version of the inflammatory bowel disease questionnaire ( IBDQ ) was administered to all patients .
	manualset3
189338	5	415510	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To quantify the impairment in the HRQOL , the 36-item version of the inflammatory bowel disease questionnaire ( IBDQ ) was administered to all patients .
	manualset3
189339	1	415511	7	NULL	NULL	0	NULL	full potential	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To realize the full potential of RT , it is essential to understand the signaling pathways that mediate inducible radiation resistance , a poorly characterized phenomenon , and identify druggable targets for radiosensitization .
	manualset3
189340	2	415511	7	NULL	NULL	0	NULL	RT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To realize the full potential of RT , it is essential to understand the signaling pathways that mediate inducible radiation resistance , a poorly characterized phenomenon , and identify druggable targets for radiosensitization .
	manualset3
189343	3	415511	7	NULL	NULL	0	NULL	signaling pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To realize the full potential of RT , it is essential to understand the signaling pathways that mediate inducible radiation resistance , a poorly characterized phenomenon , and identify druggable targets for radiosensitization .
	manualset3
189348	4	415511	7	NULL	NULL	NULL	NULL	inducible radiation resistance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To realize the full potential of RT , it is essential to understand the signaling pathways that mediate inducible radiation resistance , a poorly characterized phenomenon , and identify druggable targets for radiosensitization .
	manualset3
189351	5	415511	7	NULL	NULL	0	NULL	phenomenon	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To realize the full potential of RT , it is essential to understand the signaling pathways that mediate inducible radiation resistance , a poorly characterized phenomenon , and identify druggable targets for radiosensitization .
	manualset3
189353	6	415511	7	NULL	NULL	0	NULL	druggable targets	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To realize the full potential of RT , it is essential to understand the signaling pathways that mediate inducible radiation resistance , a poorly characterized phenomenon , and identify druggable targets for radiosensitization .
	manualset3
189354	7	415511	7	NULL	NULL	NULL	NULL	radiosensitization	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To realize the full potential of RT , it is essential to understand the signaling pathways that mediate inducible radiation resistance , a poorly characterized phenomenon , and identify druggable targets for radiosensitization .
	manualset3
189357	1	415512	7	NULL	NULL	0	NULL	flowing blood cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To recruit flowing blood cells to the inflammatory region , it would be necessary for them to interact with vascular endothelial cells .
	manualset3
189358	2	415512	7	NULL	NULL	0	NULL	 inflammatory region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To recruit flowing blood cells to the inflammatory region , it would be necessary for them to interact with vascular endothelial cells .
	manualset3
189359	3	415512	7	NULL	NULL	0	NULL	 vascular endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To recruit flowing blood cells to the inflammatory region , it would be necessary for them to interact with vascular endothelial cells .
	manualset3
189360	1	415513	7	NULL	NULL	0	NULL	imbalance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To redress this imbalance , and to encourage further temperature-dependence studies in ionic channels , we first give explicit expressions for the conductivity of ions in electrolyte solutions in terms of the microscopic parameters of the liquid .
	manualset3
189361	2	415513	7	NULL	NULL	0	NULL	temperature-dependence studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To redress this imbalance , and to encourage further temperature-dependence studies in ionic channels , we first give explicit expressions for the conductivity of ions in electrolyte solutions in terms of the microscopic parameters of the liquid .
	manualset3
189362	3	415513	7	NULL	NULL	0	NULL	ionic channels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To redress this imbalance , and to encourage further temperature-dependence studies in ionic channels , we first give explicit expressions for the conductivity of ions in electrolyte solutions in terms of the microscopic parameters of the liquid .
	manualset3
189363	4	415513	7	NULL	NULL	0	NULL	expressions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To redress this imbalance , and to encourage further temperature-dependence studies in ionic channels , we first give explicit expressions for the conductivity of ions in electrolyte solutions in terms of the microscopic parameters of the liquid .
	manualset3
189364	5	415513	7	NULL	NULL	0	NULL	conductivity of ions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To redress this imbalance , and to encourage further temperature-dependence studies in ionic channels , we first give explicit expressions for the conductivity of ions in electrolyte solutions in terms of the microscopic parameters of the liquid .
	manualset3
189365	6	415513	7	NULL	NULL	0	NULL	electrolyte solutions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To redress this imbalance , and to encourage further temperature-dependence studies in ionic channels , we first give explicit expressions for the conductivity of ions in electrolyte solutions in terms of the microscopic parameters of the liquid .
	manualset3
189366	7	415513	7	NULL	NULL	0	NULL	microscopic parameters	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	To redress this imbalance , and to encourage further temperature-dependence studies in ionic channels , we first give explicit expressions for the conductivity of ions in electrolyte solutions in terms of the microscopic parameters of the liquid .
	manualset3
189367	8	415513	7	NULL	NULL	0	NULL	liquid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To redress this imbalance , and to encourage further temperature-dependence studies in ionic channels , we first give explicit expressions for the conductivity of ions in electrolyte solutions in terms of the microscopic parameters of the liquid .
	manualset3
189368	1	415514	7	NULL	NULL	0	NULL	dimensionality	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To reduce the dimensionality , the database was resized by dividing the spectral range into four bands , and then by computing mean and standard deviation in magnitude , phase , resistance and reactance for each band and measurement .
	manualset3
189369	2	415514	7	NULL	NULL	0	NULL	database	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	To reduce the dimensionality , the database was resized by dividing the spectral range into four bands , and then by computing mean and standard deviation in magnitude , phase , resistance and reactance for each band and measurement .
	manualset3
189370	3	415514	7	NULL	NULL	0	NULL	spectral range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To reduce the dimensionality , the database was resized by dividing the spectral range into four bands , and then by computing mean and standard deviation in magnitude , phase , resistance and reactance for each band and measurement .
	manualset3
189371	4	415514	7	NULL	NULL	0	NULL	four bands	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	To reduce the dimensionality , the database was resized by dividing the spectral range into four bands , and then by computing mean and standard deviation in magnitude , phase , resistance and reactance for each band and measurement .
	manualset3
189372	5	415514	7	NULL	NULL	0	NULL	mean and standard deviation 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To reduce the dimensionality , the database was resized by dividing the spectral range into four bands , and then by computing mean and standard deviation in magnitude , phase , resistance and reactance for each band and measurement .
	manualset3
189373	6	415514	7	NULL	NULL	0	NULL	magnitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To reduce the dimensionality , the database was resized by dividing the spectral range into four bands , and then by computing mean and standard deviation in magnitude , phase , resistance and reactance for each band and measurement .
	manualset3
189374	7	415514	7	NULL	NULL	0	NULL	phase	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	To reduce the dimensionality , the database was resized by dividing the spectral range into four bands , and then by computing mean and standard deviation in magnitude , phase , resistance and reactance for each band and measurement .
	manualset3
189377	8	415514	7	NULL	NULL	0	NULL	resistance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To reduce the dimensionality , the database was resized by dividing the spectral range into four bands , and then by computing mean and standard deviation in magnitude , phase , resistance and reactance for each band and measurement .
	manualset3
189379	9	415514	7	NULL	NULL	0	NULL	reactance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To reduce the dimensionality , the database was resized by dividing the spectral range into four bands , and then by computing mean and standard deviation in magnitude , phase , resistance and reactance for each band and measurement .
	manualset3
189381	10	415514	7	NULL	NULL	0	NULL	band	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	To reduce the dimensionality , the database was resized by dividing the spectral range into four bands , and then by computing mean and standard deviation in magnitude , phase , resistance and reactance for each band and measurement .
	manualset3
189383	11	415514	7	NULL	NULL	0	NULL	measurement	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To reduce the dimensionality , the database was resized by dividing the spectral range into four bands , and then by computing mean and standard deviation in magnitude , phase , resistance and reactance for each band and measurement .
	manualset3
189386	1	415515	7	NULL	NULL	0	NULL	alliances	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To reinforce these alliances between children , as well as to prevent future peer rejection , teachers were encouraged to use cooperative , teamwork-based group activities for academic instruction .
	manualset3
189387	2	415515	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To reinforce these alliances between children , as well as to prevent future peer rejection , teachers were encouraged to use cooperative , teamwork-based group activities for academic instruction .
	manualset3
189388	3	415515	7	NULL	NULL	0	NULL	peer rejection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To reinforce these alliances between children , as well as to prevent future peer rejection , teachers were encouraged to use cooperative , teamwork-based group activities for academic instruction .
	manualset3
189389	4	415515	7	NULL	NULL	0	NULL	teachers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To reinforce these alliances between children , as well as to prevent future peer rejection , teachers were encouraged to use cooperative , teamwork-based group activities for academic instruction .
	manualset3
189390	5	415515	7	NULL	NULL	0	NULL	teamwork-based group activities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To reinforce these alliances between children , as well as to prevent future peer rejection , teachers were encouraged to use cooperative , teamwork-based group activities for academic instruction .
	manualset3
189394	6	415515	7	NULL	NULL	0	NULL	academic instruction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To reinforce these alliances between children , as well as to prevent future peer rejection , teachers were encouraged to use cooperative , teamwork-based group activities for academic instruction .
	manualset3
189404	1	415516	7	NULL	NULL	0	NULL	tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	To relate these features with tissue and mitochondrial metabolism , we studied oxygen uptake in whole isolated and perfused rat liver at two O2 supply levels , in the same liver slices , and in isolated liver mitochondria .
	manualset3
189405	2	415516	7	NULL	NULL	0	NULL	mitochondrial metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To relate these features with tissue and mitochondrial metabolism , we studied oxygen uptake in whole isolated and perfused rat liver at two O2 supply levels , in the same liver slices , and in isolated liver mitochondria .
	manualset3
189406	3	415516	7	NULL	NULL	0	NULL	oxygen uptake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To relate these features with tissue and mitochondrial metabolism , we studied oxygen uptake in whole isolated and perfused rat liver at two O2 supply levels , in the same liver slices , and in isolated liver mitochondria .
	manualset3
189407	4	415516	7	NULL	NULL	0	NULL	whole isolated and perfused rat liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To relate these features with tissue and mitochondrial metabolism , we studied oxygen uptake in whole isolated and perfused rat liver at two O2 supply levels , in the same liver slices , and in isolated liver mitochondria .
	manualset3
189408	5	415516	7	NULL	NULL	0	NULL	two O2 supply levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To relate these features with tissue and mitochondrial metabolism , we studied oxygen uptake in whole isolated and perfused rat liver at two O2 supply levels , in the same liver slices , and in isolated liver mitochondria .
	manualset3
189409	6	415516	7	NULL	NULL	0	NULL	liver slices	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To relate these features with tissue and mitochondrial metabolism , we studied oxygen uptake in whole isolated and perfused rat liver at two O2 supply levels , in the same liver slices , and in isolated liver mitochondria .
	manualset3
189410	7	415516	7	NULL	NULL	0	NULL	isolated liver mitochondria	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	To relate these features with tissue and mitochondrial metabolism , we studied oxygen uptake in whole isolated and perfused rat liver at two O2 supply levels , in the same liver slices , and in isolated liver mitochondria .
	manualset3
189549	1	415517	7	NULL	NULL	0	NULL	augmenting effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To reveal the augmenting effect of SK or shikonin on vascular endothelial growth factor ( VEGF ) production and neovascularization , we investigated murine granulomatous tissue induced by SK and shikonin , comparing them to pouches in which trehalose 6 , 6 ' - dimycolate ( TDM ) was injected .
	manualset3
189564	2	415517	7	NULL	NULL	0	NULL	SK or shikonin	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To reveal the augmenting effect of SK or shikonin on vascular endothelial growth factor ( VEGF ) production and neovascularization , we investigated murine granulomatous tissue induced by SK and shikonin , comparing them to pouches in which trehalose 6 , 6 ' - dimycolate ( TDM ) was injected .
	manualset3
189565	3	415517	7	NULL	NULL	0	NULL	vascular endothelial growth factor ( VEGF ) production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To reveal the augmenting effect of SK or shikonin on vascular endothelial growth factor ( VEGF ) production and neovascularization , we investigated murine granulomatous tissue induced by SK and shikonin , comparing them to pouches in which trehalose 6 , 6 ' - dimycolate ( TDM ) was injected .
	manualset3
189567	4	415517	7	NULL	NULL	0	NULL	neovascularization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To reveal the augmenting effect of SK or shikonin on vascular endothelial growth factor ( VEGF ) production and neovascularization , we investigated murine granulomatous tissue induced by SK and shikonin , comparing them to pouches in which trehalose 6 , 6 ' - dimycolate ( TDM ) was injected .
	manualset3
189570	5	415517	7	NULL	NULL	0	NULL	murine granulomatous tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	To reveal the augmenting effect of SK or shikonin on vascular endothelial growth factor ( VEGF ) production and neovascularization , we investigated murine granulomatous tissue induced by SK and shikonin , comparing them to pouches in which trehalose 6 , 6 ' - dimycolate ( TDM ) was injected .
	manualset3
189572	6	415517	7	NULL	NULL	0	NULL	SK	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To reveal the augmenting effect of SK or shikonin on vascular endothelial growth factor ( VEGF ) production and neovascularization , we investigated murine granulomatous tissue induced by SK and shikonin , comparing them to pouches in which trehalose 6 , 6 ' - dimycolate ( TDM ) was injected .
	manualset3
189574	7	415517	7	NULL	NULL	0	NULL	shikonin	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To reveal the augmenting effect of SK or shikonin on vascular endothelial growth factor ( VEGF ) production and neovascularization , we investigated murine granulomatous tissue induced by SK and shikonin , comparing them to pouches in which trehalose 6 , 6 ' - dimycolate ( TDM ) was injected .
	manualset3
189577	8	415517	7	NULL	NULL	0	NULL	pouches	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	To reveal the augmenting effect of SK or shikonin on vascular endothelial growth factor ( VEGF ) production and neovascularization , we investigated murine granulomatous tissue induced by SK and shikonin , comparing them to pouches in which trehalose 6 , 6 ' - dimycolate ( TDM ) was injected .
	manualset3
189579	9	415517	7	NULL	NULL	0	NULL	trehalose 6 , 6 ' - dimycolate ( TDM )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To reveal the augmenting effect of SK or shikonin on vascular endothelial growth factor ( VEGF ) production and neovascularization , we investigated murine granulomatous tissue induced by SK and shikonin , comparing them to pouches in which trehalose 6 , 6 ' - dimycolate ( TDM ) was injected .
	manualset3
189587	1	415518	7	NULL	NULL	0	NULL	resealing process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To simulate resealing process , Gpore was assumed to decrease after the shock exponentially at a time constant ( tau pore ) of 5-50 s. The simulation results are qualitatively consistent with our experimental observations in guinea pig papillary muscle ( 1 ) ; they include prolonged depolarization , diastolic depolarization or oscillation of membrane potential leading to a single or multiple spontaneous excitation .
	manualset3
189615	2	415518	7	NULL	NULL	0	NULL	Gpore	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To simulate resealing process , Gpore was assumed to decrease after the shock exponentially at a time constant ( tau pore ) of 5-50 s. The simulation results are qualitatively consistent with our experimental observations in guinea pig papillary muscle ( 1 ) ; they include prolonged depolarization , diastolic depolarization or oscillation of membrane potential leading to a single or multiple spontaneous excitation .
	manualset3
189619	3	415518	7	NULL	NULL	0	NULL	shock	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	To simulate resealing process , Gpore was assumed to decrease after the shock exponentially at a time constant ( tau pore ) of 5-50 s. The simulation results are qualitatively consistent with our experimental observations in guinea pig papillary muscle ( 1 ) ; they include prolonged depolarization , diastolic depolarization or oscillation of membrane potential leading to a single or multiple spontaneous excitation .
	manualset3
189622	4	415518	7	NULL	NULL	0	NULL	time constant ( tau pore ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To simulate resealing process , Gpore was assumed to decrease after the shock exponentially at a time constant ( tau pore ) of 5-50 s. The simulation results are qualitatively consistent with our experimental observations in guinea pig papillary muscle ( 1 ) ; they include prolonged depolarization , diastolic depolarization or oscillation of membrane potential leading to a single or multiple spontaneous excitation .
	manualset3
189625	5	415518	7	NULL	NULL	0	NULL	5-50 s	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	To simulate resealing process , Gpore was assumed to decrease after the shock exponentially at a time constant ( tau pore ) of 5-50 s. The simulation results are qualitatively consistent with our experimental observations in guinea pig papillary muscle ( 1 ) ; they include prolonged depolarization , diastolic depolarization or oscillation of membrane potential leading to a single or multiple spontaneous excitation .
	manualset3
189629	6	415518	7	NULL	NULL	0	NULL	 simulation results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To simulate resealing process , Gpore was assumed to decrease after the shock exponentially at a time constant ( tau pore ) of 5-50 s. The simulation results are qualitatively consistent with our experimental observations in guinea pig papillary muscle ( 1 ) ; they include prolonged depolarization , diastolic depolarization or oscillation of membrane potential leading to a single or multiple spontaneous excitation .
	manualset3
189631	7	415518	7	NULL	NULL	0	NULL	experimental observations	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	To simulate resealing process , Gpore was assumed to decrease after the shock exponentially at a time constant ( tau pore ) of 5-50 s. The simulation results are qualitatively consistent with our experimental observations in guinea pig papillary muscle ( 1 ) ; they include prolonged depolarization , diastolic depolarization or oscillation of membrane potential leading to a single or multiple spontaneous excitation .
	manualset3
189651	8	415518	7	NULL	NULL	0	NULL	guinea pig papillary muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To simulate resealing process , Gpore was assumed to decrease after the shock exponentially at a time constant ( tau pore ) of 5-50 s. The simulation results are qualitatively consistent with our experimental observations in guinea pig papillary muscle ( 1 ) ; they include prolonged depolarization , diastolic depolarization or oscillation of membrane potential leading to a single or multiple spontaneous excitation .
	manualset3
189652	9	415518	7	NULL	NULL	0	NULL	prolonged depolarization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To simulate resealing process , Gpore was assumed to decrease after the shock exponentially at a time constant ( tau pore ) of 5-50 s. The simulation results are qualitatively consistent with our experimental observations in guinea pig papillary muscle ( 1 ) ; they include prolonged depolarization , diastolic depolarization or oscillation of membrane potential leading to a single or multiple spontaneous excitation .
	manualset3
189655	10	415518	7	NULL	NULL	0	NULL	diastolic depolarization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To simulate resealing process , Gpore was assumed to decrease after the shock exponentially at a time constant ( tau pore ) of 5-50 s. The simulation results are qualitatively consistent with our experimental observations in guinea pig papillary muscle ( 1 ) ; they include prolonged depolarization , diastolic depolarization or oscillation of membrane potential leading to a single or multiple spontaneous excitation .
	manualset3
189658	11	415518	7	NULL	NULL	0	NULL	oscillation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To simulate resealing process , Gpore was assumed to decrease after the shock exponentially at a time constant ( tau pore ) of 5-50 s. The simulation results are qualitatively consistent with our experimental observations in guinea pig papillary muscle ( 1 ) ; they include prolonged depolarization , diastolic depolarization or oscillation of membrane potential leading to a single or multiple spontaneous excitation .
	manualset3
189659	12	415518	7	NULL	NULL	0	NULL	membrane potential	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To simulate resealing process , Gpore was assumed to decrease after the shock exponentially at a time constant ( tau pore ) of 5-50 s. The simulation results are qualitatively consistent with our experimental observations in guinea pig papillary muscle ( 1 ) ; they include prolonged depolarization , diastolic depolarization or oscillation of membrane potential leading to a single or multiple spontaneous excitation .
	manualset3
189660	13	415518	7	NULL	NULL	0	NULL	single or multiple spontaneous excitation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To simulate resealing process , Gpore was assumed to decrease after the shock exponentially at a time constant ( tau pore ) of 5-50 s. The simulation results are qualitatively consistent with our experimental observations in guinea pig papillary muscle ( 1 ) ; they include prolonged depolarization , diastolic depolarization or oscillation of membrane potential leading to a single or multiple spontaneous excitation .
	manualset3
189661	1	415519	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	To study a relationship between the skull base and cervical spine anomalies and Chiari type I malformation ( CMI ) , 364 patients with CMI were examined using craniography and magnetic resonance imaging of the brain and spinal cord .
	manualset3
189662	2	415519	7	NULL	NULL	0	NULL	skull base	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To study a relationship between the skull base and cervical spine anomalies and Chiari type I malformation ( CMI ) , 364 patients with CMI were examined using craniography and magnetic resonance imaging of the brain and spinal cord .
	manualset3
189663	3	415519	7	NULL	NULL	0	NULL	cervical spine anomalies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To study a relationship between the skull base and cervical spine anomalies and Chiari type I malformation ( CMI ) , 364 patients with CMI were examined using craniography and magnetic resonance imaging of the brain and spinal cord .
	manualset3
189664	4	415519	7	NULL	NULL	0	NULL	Chiari type I malformation ( CMI )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To study a relationship between the skull base and cervical spine anomalies and Chiari type I malformation ( CMI ) , 364 patients with CMI were examined using craniography and magnetic resonance imaging of the brain and spinal cord .
	manualset3
189665	5	415519	7	NULL	NULL	0	NULL	364 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To study a relationship between the skull base and cervical spine anomalies and Chiari type I malformation ( CMI ) , 364 patients with CMI were examined using craniography and magnetic resonance imaging of the brain and spinal cord .
	manualset3
189666	6	415519	7	NULL	NULL	0	NULL	CMI 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To study a relationship between the skull base and cervical spine anomalies and Chiari type I malformation ( CMI ) , 364 patients with CMI were examined using craniography and magnetic resonance imaging of the brain and spinal cord .
	manualset3
189667	7	415519	7	NULL	NULL	0	NULL	craniography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To study a relationship between the skull base and cervical spine anomalies and Chiari type I malformation ( CMI ) , 364 patients with CMI were examined using craniography and magnetic resonance imaging of the brain and spinal cord .
	manualset3
189668	8	415519	7	NULL	NULL	NULL	NULL	magnetic resonance imaging	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To study a relationship between the skull base and cervical spine anomalies and Chiari type I malformation ( CMI ) , 364 patients with CMI were examined using craniography and magnetic resonance imaging of the brain and spinal cord .
	manualset3
189669	9	415519	7	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To study a relationship between the skull base and cervical spine anomalies and Chiari type I malformation ( CMI ) , 364 patients with CMI were examined using craniography and magnetic resonance imaging of the brain and spinal cord .
	manualset3
189670	10	415519	7	NULL	NULL	0	NULL	spinal cord	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To study a relationship between the skull base and cervical spine anomalies and Chiari type I malformation ( CMI ) , 364 patients with CMI were examined using craniography and magnetic resonance imaging of the brain and spinal cord .
	manualset3
189671	1	415520	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	To study the relationship between duck hepatitis B virus ( DHBV ) infection and duck hepatocellular carcinoma ( DHCC ) , histological examination and DHBV DNA hybridization were performed in 875 ducks from three flocks in Qidong County .
	manualset3
189672	2	415520	7	NULL	NULL	0	NULL	duck hepatitis B virus ( DHBV ) infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To study the relationship between duck hepatitis B virus ( DHBV ) infection and duck hepatocellular carcinoma ( DHCC ) , histological examination and DHBV DNA hybridization were performed in 875 ducks from three flocks in Qidong County .
	manualset3
189673	3	415520	7	NULL	NULL	0	NULL	duck hepatocellular carcinoma ( DHCC )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To study the relationship between duck hepatitis B virus ( DHBV ) infection and duck hepatocellular carcinoma ( DHCC ) , histological examination and DHBV DNA hybridization were performed in 875 ducks from three flocks in Qidong County .
	manualset3
189675	4	415520	7	NULL	NULL	0	NULL	histological examination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To study the relationship between duck hepatitis B virus ( DHBV ) infection and duck hepatocellular carcinoma ( DHCC ) , histological examination and DHBV DNA hybridization were performed in 875 ducks from three flocks in Qidong County .
	manualset3
189676	5	415520	7	NULL	NULL	0	NULL	DHBV DNA hybridization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To study the relationship between duck hepatitis B virus ( DHBV ) infection and duck hepatocellular carcinoma ( DHCC ) , histological examination and DHBV DNA hybridization were performed in 875 ducks from three flocks in Qidong County .
	manualset3
189677	6	415520	7	NULL	NULL	0	NULL	875 ducks	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To study the relationship between duck hepatitis B virus ( DHBV ) infection and duck hepatocellular carcinoma ( DHCC ) , histological examination and DHBV DNA hybridization were performed in 875 ducks from three flocks in Qidong County .
	manualset3
189678	7	415520	7	NULL	NULL	0	NULL	three flocks	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To study the relationship between duck hepatitis B virus ( DHBV ) infection and duck hepatocellular carcinoma ( DHCC ) , histological examination and DHBV DNA hybridization were performed in 875 ducks from three flocks in Qidong County .
	manualset3
189679	8	415520	7	NULL	NULL	0	NULL	Qidong County 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	To study the relationship between duck hepatitis B virus ( DHBV ) infection and duck hepatocellular carcinoma ( DHCC ) , histological examination and DHBV DNA hybridization were performed in 875 ducks from three flocks in Qidong County .
	manualset3
189680	1	415521	7	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	To support this hypothesis , we investigated whether two other cationic proteins , platelet factor 4 ( PF4 ) and cathepsin G , were capable of inducing AHR .
	manualset3
189681	2	415521	7	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To support this hypothesis , we investigated whether two other cationic proteins , platelet factor 4 ( PF4 ) and cathepsin G , were capable of inducing AHR .
	manualset3
189682	3	415521	7	NULL	NULL	0	NULL	cationic proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To support this hypothesis , we investigated whether two other cationic proteins , platelet factor 4 ( PF4 ) and cathepsin G , were capable of inducing AHR .
	manualset3
189683	4	415521	7	NULL	NULL	0	NULL	platelet factor 4 ( PF4 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To support this hypothesis , we investigated whether two other cationic proteins , platelet factor 4 ( PF4 ) and cathepsin G , were capable of inducing AHR .
	manualset3
189684	5	415521	7	NULL	NULL	0	NULL	cathepsin G	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To support this hypothesis , we investigated whether two other cationic proteins , platelet factor 4 ( PF4 ) and cathepsin G , were capable of inducing AHR .
	manualset3
189685	6	415521	7	NULL	NULL	0	NULL	inducing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To support this hypothesis , we investigated whether two other cationic proteins , platelet factor 4 ( PF4 ) and cathepsin G , were capable of inducing AHR .
	manualset3
189686	7	415521	7	NULL	NULL	0	NULL	AHR	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To support this hypothesis , we investigated whether two other cationic proteins , platelet factor 4 ( PF4 ) and cathepsin G , were capable of inducing AHR .
	manualset3
189687	1	415522	7	NULL	NULL	NULL	NULL	homology model scoring procedure	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To test our homology model scoring procedure for various amino acid labeling schemes , we generated a library of 7 , 474 homology models for 22 protein targets culled from the TALOS + / SPARTA + training set of protein structures .
	manualset3
189688	2	415522	7	NULL	NULL	0	NULL	amino acid labeling schemes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To test our homology model scoring procedure for various amino acid labeling schemes , we generated a library of 7 , 474 homology models for 22 protein targets culled from the TALOS + / SPARTA + training set of protein structures .
	manualset3
189689	3	415522	7	NULL	NULL	0	NULL	 library 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	To test our homology model scoring procedure for various amino acid labeling schemes , we generated a library of 7 , 474 homology models for 22 protein targets culled from the TALOS + / SPARTA + training set of protein structures .
	manualset3
189690	4	415522	7	NULL	NULL	NULL	NULL	7 , 474 homology models	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To test our homology model scoring procedure for various amino acid labeling schemes , we generated a library of 7 , 474 homology models for 22 protein targets culled from the TALOS + / SPARTA + training set of protein structures .
	manualset3
189691	5	415522	7	NULL	NULL	0	NULL	22 protein targets	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To test our homology model scoring procedure for various amino acid labeling schemes , we generated a library of 7 , 474 homology models for 22 protein targets culled from the TALOS + / SPARTA + training set of protein structures .
	manualset3
189692	6	415522	7	NULL	NULL	0	NULL	TALOS + / SPARTA + training set	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	To test our homology model scoring procedure for various amino acid labeling schemes , we generated a library of 7 , 474 homology models for 22 protein targets culled from the TALOS + / SPARTA + training set of protein structures .
	manualset3
189693	7	415522	7	NULL	NULL	0	NULL	protein structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To test our homology model scoring procedure for various amino acid labeling schemes , we generated a library of 7 , 474 homology models for 22 protein targets culled from the TALOS + / SPARTA + training set of protein structures .
	manualset3
189694	1	415523	7	NULL	NULL	0	NULL	day 15	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	After day 15 , 10 % of patients died from treatment-related complications with infection as the main cause of death .
	manualset3
189695	2	415523	7	NULL	NULL	0	NULL	10 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After day 15 , 10 % of patients died from treatment-related complications with infection as the main cause of death .
	manualset3
189696	3	415523	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	After day 15 , 10 % of patients died from treatment-related complications with infection as the main cause of death .
	manualset3
189697	4	415523	7	NULL	NULL	0	NULL	treatment-related complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After day 15 , 10 % of patients died from treatment-related complications with infection as the main cause of death .
	manualset3
189698	5	415523	7	NULL	NULL	0	NULL	infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After day 15 , 10 % of patients died from treatment-related complications with infection as the main cause of death .
	manualset3
189699	6	415523	7	NULL	NULL	0	NULL	death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After day 15 , 10 % of patients died from treatment-related complications with infection as the main cause of death .
	manualset3
189700	1	415524	7	NULL	NULL	0	NULL	 protein 's nuclear targeting ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To test the protein 's nuclear targeting ability , SubH2Bv , with and without targeted mutations of the basic residues of bNLS , as well as bNLS alone , were transfected into mammalian cells as GFP-fusion proteins .
	manualset3
189701	2	415524	7	NULL	NULL	0	NULL	SubH2Bv	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To test the protein 's nuclear targeting ability , SubH2Bv , with and without targeted mutations of the basic residues of bNLS , as well as bNLS alone , were transfected into mammalian cells as GFP-fusion proteins .
	manualset3
189702	3	415524	7	NULL	NULL	0	NULL	targeted mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To test the protein 's nuclear targeting ability , SubH2Bv , with and without targeted mutations of the basic residues of bNLS , as well as bNLS alone , were transfected into mammalian cells as GFP-fusion proteins .
	manualset3
189703	4	415524	7	NULL	NULL	0	NULL	basic residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To test the protein 's nuclear targeting ability , SubH2Bv , with and without targeted mutations of the basic residues of bNLS , as well as bNLS alone , were transfected into mammalian cells as GFP-fusion proteins .
	manualset3
189704	5	415524	7	NULL	NULL	0	NULL	bNLS	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To test the protein 's nuclear targeting ability , SubH2Bv , with and without targeted mutations of the basic residues of bNLS , as well as bNLS alone , were transfected into mammalian cells as GFP-fusion proteins .
	manualset3
189705	6	415524	7	NULL	NULL	0	NULL	bNLS	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To test the protein 's nuclear targeting ability , SubH2Bv , with and without targeted mutations of the basic residues of bNLS , as well as bNLS alone , were transfected into mammalian cells as GFP-fusion proteins .
	manualset3
189706	7	415524	7	NULL	NULL	0	NULL	mammalian cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To test the protein 's nuclear targeting ability , SubH2Bv , with and without targeted mutations of the basic residues of bNLS , as well as bNLS alone , were transfected into mammalian cells as GFP-fusion proteins .
	manualset3
189707	8	415524	7	NULL	NULL	0	NULL	GFP-fusion proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To test the protein 's nuclear targeting ability , SubH2Bv , with and without targeted mutations of the basic residues of bNLS , as well as bNLS alone , were transfected into mammalian cells as GFP-fusion proteins .
	manualset3
189708	1	415525	7	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , a frog ( Xenopus tropicalis ) MC2R was expressed in CHO cells either in the presence of a tetrapod ( mouse ) MRAP1 or a bony fish ( zebrafish ) MRAP1 .
	manualset3
189709	2	415525	7	NULL	NULL	NULL	NULL	frog ( Xenopus tropicalis ) MC2R	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , a frog ( Xenopus tropicalis ) MC2R was expressed in CHO cells either in the presence of a tetrapod ( mouse ) MRAP1 or a bony fish ( zebrafish ) MRAP1 .
	manualset3
189711	4	415525	7	NULL	NULL	0	NULL	CHO cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , a frog ( Xenopus tropicalis ) MC2R was expressed in CHO cells either in the presence of a tetrapod ( mouse ) MRAP1 or a bony fish ( zebrafish ) MRAP1 .
	manualset3
189712	5	415525	7	NULL	NULL	0	NULL	tetrapod ( mouse ) MRAP1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , a frog ( Xenopus tropicalis ) MC2R was expressed in CHO cells either in the presence of a tetrapod ( mouse ) MRAP1 or a bony fish ( zebrafish ) MRAP1 .
	manualset3
189713	6	415525	7	NULL	NULL	0	NULL	 bony fish ( zebrafish ) MRAP1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , a frog ( Xenopus tropicalis ) MC2R was expressed in CHO cells either in the presence of a tetrapod ( mouse ) MRAP1 or a bony fish ( zebrafish ) MRAP1 .
	manualset3
189714	1	415526	7	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , adult male Sprague Dawley rats received moderate parasagittal fluid-percussion brain injury , and were then maintained at normothermic or moderate hypothermic temperatures for 4 h. At 12 weeks after recovery , seizure susceptibility was assessed by challenging the animals with pentylenetetrazole , a GABA ( A ) receptor antagonist .
	manualset3
189715	2	415526	7	NULL	NULL	0	NULL	 adult male Sprague Dawley rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , adult male Sprague Dawley rats received moderate parasagittal fluid-percussion brain injury , and were then maintained at normothermic or moderate hypothermic temperatures for 4 h. At 12 weeks after recovery , seizure susceptibility was assessed by challenging the animals with pentylenetetrazole , a GABA ( A ) receptor antagonist .
	manualset3
189716	3	415526	7	NULL	NULL	0	NULL	moderate parasagittal fluid-percussion brain injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , adult male Sprague Dawley rats received moderate parasagittal fluid-percussion brain injury , and were then maintained at normothermic or moderate hypothermic temperatures for 4 h. At 12 weeks after recovery , seizure susceptibility was assessed by challenging the animals with pentylenetetrazole , a GABA ( A ) receptor antagonist .
	manualset3
189717	4	415526	7	NULL	NULL	0	NULL	normothermic temperatures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , adult male Sprague Dawley rats received moderate parasagittal fluid-percussion brain injury , and were then maintained at normothermic or moderate hypothermic temperatures for 4 h. At 12 weeks after recovery , seizure susceptibility was assessed by challenging the animals with pentylenetetrazole , a GABA ( A ) receptor antagonist .
	manualset3
189718	5	415526	7	NULL	NULL	0	NULL	moderate hypothermic temperatures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , adult male Sprague Dawley rats received moderate parasagittal fluid-percussion brain injury , and were then maintained at normothermic or moderate hypothermic temperatures for 4 h. At 12 weeks after recovery , seizure susceptibility was assessed by challenging the animals with pentylenetetrazole , a GABA ( A ) receptor antagonist .
	manualset3
189719	6	415526	7	NULL	NULL	0	NULL	4 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , adult male Sprague Dawley rats received moderate parasagittal fluid-percussion brain injury , and were then maintained at normothermic or moderate hypothermic temperatures for 4 h. At 12 weeks after recovery , seizure susceptibility was assessed by challenging the animals with pentylenetetrazole , a GABA ( A ) receptor antagonist .
	manualset3
189720	7	415526	7	NULL	NULL	0	NULL	12 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , adult male Sprague Dawley rats received moderate parasagittal fluid-percussion brain injury , and were then maintained at normothermic or moderate hypothermic temperatures for 4 h. At 12 weeks after recovery , seizure susceptibility was assessed by challenging the animals with pentylenetetrazole , a GABA ( A ) receptor antagonist .
	manualset3
189721	8	415526	7	NULL	NULL	0	NULL	recovery 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , adult male Sprague Dawley rats received moderate parasagittal fluid-percussion brain injury , and were then maintained at normothermic or moderate hypothermic temperatures for 4 h. At 12 weeks after recovery , seizure susceptibility was assessed by challenging the animals with pentylenetetrazole , a GABA ( A ) receptor antagonist .
	manualset3
189722	9	415526	7	NULL	NULL	0	NULL	seizure susceptibility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , adult male Sprague Dawley rats received moderate parasagittal fluid-percussion brain injury , and were then maintained at normothermic or moderate hypothermic temperatures for 4 h. At 12 weeks after recovery , seizure susceptibility was assessed by challenging the animals with pentylenetetrazole , a GABA ( A ) receptor antagonist .
	manualset3
189723	10	415526	7	NULL	NULL	0	NULL	challenging	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , adult male Sprague Dawley rats received moderate parasagittal fluid-percussion brain injury , and were then maintained at normothermic or moderate hypothermic temperatures for 4 h. At 12 weeks after recovery , seizure susceptibility was assessed by challenging the animals with pentylenetetrazole , a GABA ( A ) receptor antagonist .
	manualset3
189724	11	415526	7	NULL	NULL	0	NULL	 animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , adult male Sprague Dawley rats received moderate parasagittal fluid-percussion brain injury , and were then maintained at normothermic or moderate hypothermic temperatures for 4 h. At 12 weeks after recovery , seizure susceptibility was assessed by challenging the animals with pentylenetetrazole , a GABA ( A ) receptor antagonist .
	manualset3
189725	12	415526	7	NULL	NULL	0	NULL	 pentylenetetrazole	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , adult male Sprague Dawley rats received moderate parasagittal fluid-percussion brain injury , and were then maintained at normothermic or moderate hypothermic temperatures for 4 h. At 12 weeks after recovery , seizure susceptibility was assessed by challenging the animals with pentylenetetrazole , a GABA ( A ) receptor antagonist .
	manualset3
189726	13	415526	7	NULL	NULL	0	NULL	GABA ( A ) receptor antagonist 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , adult male Sprague Dawley rats received moderate parasagittal fluid-percussion brain injury , and were then maintained at normothermic or moderate hypothermic temperatures for 4 h. At 12 weeks after recovery , seizure susceptibility was assessed by challenging the animals with pentylenetetrazole , a GABA ( A ) receptor antagonist .
	manualset3
189727	1	415527	7	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , p50-knockout and wild-type ( WT ) mice were exposed to CS for 3 days to 6 mo , and inflammatory responses as well as air space enlargement were assessed .
	manualset3
189728	2	415527	7	NULL	NULL	0	NULL	p50-knockout mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , p50-knockout and wild-type ( WT ) mice were exposed to CS for 3 days to 6 mo , and inflammatory responses as well as air space enlargement were assessed .
	manualset3
189729	3	415527	7	NULL	NULL	0	NULL	wild-type ( WT ) mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , p50-knockout and wild-type ( WT ) mice were exposed to CS for 3 days to 6 mo , and inflammatory responses as well as air space enlargement were assessed .
	manualset3
189730	4	415527	7	NULL	NULL	0	NULL	CS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , p50-knockout and wild-type ( WT ) mice were exposed to CS for 3 days to 6 mo , and inflammatory responses as well as air space enlargement were assessed .
	manualset3
189731	5	415527	7	NULL	NULL	0	NULL	3 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , p50-knockout and wild-type ( WT ) mice were exposed to CS for 3 days to 6 mo , and inflammatory responses as well as air space enlargement were assessed .
	manualset3
189732	6	415527	7	NULL	NULL	0	NULL	6 mo	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , p50-knockout and wild-type ( WT ) mice were exposed to CS for 3 days to 6 mo , and inflammatory responses as well as air space enlargement were assessed .
	manualset3
189733	7	415527	7	NULL	NULL	NULL	NULL	inflammatory responses	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , p50-knockout and wild-type ( WT ) mice were exposed to CS for 3 days to 6 mo , and inflammatory responses as well as air space enlargement were assessed .
	manualset3
189734	8	415527	7	NULL	NULL	0	NULL	air space enlargement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , p50-knockout and wild-type ( WT ) mice were exposed to CS for 3 days to 6 mo , and inflammatory responses as well as air space enlargement were assessed .
	manualset3
189735	1	415528	7	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , we measured indexes of platelet activation ( soluble P-selectin ) , endothelial damage or dysfunction ( von Willebrand factor ( vWf ) , enzyme-linked immunosorbent assay ) and fibrinogen ( modified Clauss ) in 56 consecutive patients ( 35 women , mean age 65 years ) admitted for isolated mitral valve repair ( n = 39 ) or replacement ( using mechanical implants , n = 17 ) .
	manualset3
189736	2	415528	7	NULL	NULL	0	NULL	indexes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , we measured indexes of platelet activation ( soluble P-selectin ) , endothelial damage or dysfunction ( von Willebrand factor ( vWf ) , enzyme-linked immunosorbent assay ) and fibrinogen ( modified Clauss ) in 56 consecutive patients ( 35 women , mean age 65 years ) admitted for isolated mitral valve repair ( n = 39 ) or replacement ( using mechanical implants , n = 17 ) .
	manualset3
189737	3	415528	7	NULL	NULL	0	NULL	platelet activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , we measured indexes of platelet activation ( soluble P-selectin ) , endothelial damage or dysfunction ( von Willebrand factor ( vWf ) , enzyme-linked immunosorbent assay ) and fibrinogen ( modified Clauss ) in 56 consecutive patients ( 35 women , mean age 65 years ) admitted for isolated mitral valve repair ( n = 39 ) or replacement ( using mechanical implants , n = 17 ) .
	manualset3
189738	4	415528	7	NULL	NULL	0	NULL	soluble P-selectin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , we measured indexes of platelet activation ( soluble P-selectin ) , endothelial damage or dysfunction ( von Willebrand factor ( vWf ) , enzyme-linked immunosorbent assay ) and fibrinogen ( modified Clauss ) in 56 consecutive patients ( 35 women , mean age 65 years ) admitted for isolated mitral valve repair ( n = 39 ) or replacement ( using mechanical implants , n = 17 ) .
	manualset3
189739	5	415528	7	NULL	NULL	NULL	NULL	endothelial damage 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , we measured indexes of platelet activation ( soluble P-selectin ) , endothelial damage or dysfunction ( von Willebrand factor ( vWf ) , enzyme-linked immunosorbent assay ) and fibrinogen ( modified Clauss ) in 56 consecutive patients ( 35 women , mean age 65 years ) admitted for isolated mitral valve repair ( n = 39 ) or replacement ( using mechanical implants , n = 17 ) .
	manualset3
189740	6	415528	7	NULL	NULL	NULL	NULL	dysfunction	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , we measured indexes of platelet activation ( soluble P-selectin ) , endothelial damage or dysfunction ( von Willebrand factor ( vWf ) , enzyme-linked immunosorbent assay ) and fibrinogen ( modified Clauss ) in 56 consecutive patients ( 35 women , mean age 65 years ) admitted for isolated mitral valve repair ( n = 39 ) or replacement ( using mechanical implants , n = 17 ) .
	manualset3
189741	7	415528	7	NULL	NULL	0	NULL	von Willebrand factor ( vWf )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , we measured indexes of platelet activation ( soluble P-selectin ) , endothelial damage or dysfunction ( von Willebrand factor ( vWf ) , enzyme-linked immunosorbent assay ) and fibrinogen ( modified Clauss ) in 56 consecutive patients ( 35 women , mean age 65 years ) admitted for isolated mitral valve repair ( n = 39 ) or replacement ( using mechanical implants , n = 17 ) .
	manualset3
189742	8	415528	7	NULL	NULL	0	NULL	enzyme-linked immunosorbent assay ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , we measured indexes of platelet activation ( soluble P-selectin ) , endothelial damage or dysfunction ( von Willebrand factor ( vWf ) , enzyme-linked immunosorbent assay ) and fibrinogen ( modified Clauss ) in 56 consecutive patients ( 35 women , mean age 65 years ) admitted for isolated mitral valve repair ( n = 39 ) or replacement ( using mechanical implants , n = 17 ) .
	manualset3
189743	9	415528	7	NULL	NULL	0	NULL	fibrinogen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , we measured indexes of platelet activation ( soluble P-selectin ) , endothelial damage or dysfunction ( von Willebrand factor ( vWf ) , enzyme-linked immunosorbent assay ) and fibrinogen ( modified Clauss ) in 56 consecutive patients ( 35 women , mean age 65 years ) admitted for isolated mitral valve repair ( n = 39 ) or replacement ( using mechanical implants , n = 17 ) .
	manualset3
189744	10	415528	7	NULL	NULL	0	NULL	modified Clauss	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , we measured indexes of platelet activation ( soluble P-selectin ) , endothelial damage or dysfunction ( von Willebrand factor ( vWf ) , enzyme-linked immunosorbent assay ) and fibrinogen ( modified Clauss ) in 56 consecutive patients ( 35 women , mean age 65 years ) admitted for isolated mitral valve repair ( n = 39 ) or replacement ( using mechanical implants , n = 17 ) .
	manualset3
189745	11	415528	7	NULL	NULL	0	NULL	56 consecutive patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , we measured indexes of platelet activation ( soluble P-selectin ) , endothelial damage or dysfunction ( von Willebrand factor ( vWf ) , enzyme-linked immunosorbent assay ) and fibrinogen ( modified Clauss ) in 56 consecutive patients ( 35 women , mean age 65 years ) admitted for isolated mitral valve repair ( n = 39 ) or replacement ( using mechanical implants , n = 17 ) .
	manualset3
189746	12	415528	7	NULL	NULL	0	NULL	35 women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , we measured indexes of platelet activation ( soluble P-selectin ) , endothelial damage or dysfunction ( von Willebrand factor ( vWf ) , enzyme-linked immunosorbent assay ) and fibrinogen ( modified Clauss ) in 56 consecutive patients ( 35 women , mean age 65 years ) admitted for isolated mitral valve repair ( n = 39 ) or replacement ( using mechanical implants , n = 17 ) .
	manualset3
189747	13	415528	7	NULL	NULL	0	NULL	mean age 65 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , we measured indexes of platelet activation ( soluble P-selectin ) , endothelial damage or dysfunction ( von Willebrand factor ( vWf ) , enzyme-linked immunosorbent assay ) and fibrinogen ( modified Clauss ) in 56 consecutive patients ( 35 women , mean age 65 years ) admitted for isolated mitral valve repair ( n = 39 ) or replacement ( using mechanical implants , n = 17 ) .
	manualset3
189748	14	415528	7	NULL	NULL	0	NULL	isolated mitral valve repair	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , we measured indexes of platelet activation ( soluble P-selectin ) , endothelial damage or dysfunction ( von Willebrand factor ( vWf ) , enzyme-linked immunosorbent assay ) and fibrinogen ( modified Clauss ) in 56 consecutive patients ( 35 women , mean age 65 years ) admitted for isolated mitral valve repair ( n = 39 ) or replacement ( using mechanical implants , n = 17 ) .
	manualset3
189749	15	415528	7	NULL	NULL	0	NULL	n = 39 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , we measured indexes of platelet activation ( soluble P-selectin ) , endothelial damage or dysfunction ( von Willebrand factor ( vWf ) , enzyme-linked immunosorbent assay ) and fibrinogen ( modified Clauss ) in 56 consecutive patients ( 35 women , mean age 65 years ) admitted for isolated mitral valve repair ( n = 39 ) or replacement ( using mechanical implants , n = 17 ) .
	manualset3
189750	16	415528	7	NULL	NULL	0	NULL	replacement	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , we measured indexes of platelet activation ( soluble P-selectin ) , endothelial damage or dysfunction ( von Willebrand factor ( vWf ) , enzyme-linked immunosorbent assay ) and fibrinogen ( modified Clauss ) in 56 consecutive patients ( 35 women , mean age 65 years ) admitted for isolated mitral valve repair ( n = 39 ) or replacement ( using mechanical implants , n = 17 ) .
	manualset3
189751	17	415528	7	NULL	NULL	0	NULL	mechanical implants	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , we measured indexes of platelet activation ( soluble P-selectin ) , endothelial damage or dysfunction ( von Willebrand factor ( vWf ) , enzyme-linked immunosorbent assay ) and fibrinogen ( modified Clauss ) in 56 consecutive patients ( 35 women , mean age 65 years ) admitted for isolated mitral valve repair ( n = 39 ) or replacement ( using mechanical implants , n = 17 ) .
	manualset3
189752	18	415528	7	NULL	NULL	0	NULL	n = 17 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this hypothesis , we measured indexes of platelet activation ( soluble P-selectin ) , endothelial damage or dysfunction ( von Willebrand factor ( vWf ) , enzyme-linked immunosorbent assay ) and fibrinogen ( modified Clauss ) in 56 consecutive patients ( 35 women , mean age 65 years ) admitted for isolated mitral valve repair ( n = 39 ) or replacement ( using mechanical implants , n = 17 ) .
	manualset3
189753	1	415529	7	NULL	NULL	0	NULL	pattern	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this pattern in non-mammal herbivores , we conducted feeding trails with 24 tortoises of various species ( M range 0.52-180 kg ) fed a diet of grass hay ad libitum and salad .
	manualset3
189754	2	415529	7	NULL	NULL	0	NULL	non-mammal herbivores	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this pattern in non-mammal herbivores , we conducted feeding trails with 24 tortoises of various species ( M range 0.52-180 kg ) fed a diet of grass hay ad libitum and salad .
	manualset3
189755	3	415529	7	NULL	NULL	0	NULL	feeding trails	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this pattern in non-mammal herbivores , we conducted feeding trails with 24 tortoises of various species ( M range 0.52-180 kg ) fed a diet of grass hay ad libitum and salad .
	manualset3
189756	4	415529	7	NULL	NULL	0	NULL	24 tortoises 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this pattern in non-mammal herbivores , we conducted feeding trails with 24 tortoises of various species ( M range 0.52-180 kg ) fed a diet of grass hay ad libitum and salad .
	manualset3
189757	5	415529	7	NULL	NULL	0	NULL	species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this pattern in non-mammal herbivores , we conducted feeding trails with 24 tortoises of various species ( M range 0.52-180 kg ) fed a diet of grass hay ad libitum and salad .
	manualset3
189758	6	415529	7	NULL	NULL	0	NULL	M range 0.52-180 kg 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this pattern in non-mammal herbivores , we conducted feeding trails with 24 tortoises of various species ( M range 0.52-180 kg ) fed a diet of grass hay ad libitum and salad .
	manualset3
189759	7	415529	7	NULL	NULL	0	NULL	diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this pattern in non-mammal herbivores , we conducted feeding trails with 24 tortoises of various species ( M range 0.52-180 kg ) fed a diet of grass hay ad libitum and salad .
	manualset3
189760	8	415529	7	NULL	NULL	0	NULL	 grass hay ad libitum	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this pattern in non-mammal herbivores , we conducted feeding trails with 24 tortoises of various species ( M range 0.52-180 kg ) fed a diet of grass hay ad libitum and salad .
	manualset3
189761	9	415529	7	NULL	NULL	0	NULL	salad	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	To test this pattern in non-mammal herbivores , we conducted feeding trails with 24 tortoises of various species ( M range 0.52-180 kg ) fed a diet of grass hay ad libitum and salad .
	manualset3
189762	1	415530	7	NULL	NULL	0	NULL	distal tubular injections ( 14C )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After distal tubular injections ( 14C ) glucose recovery was complete in both C and VE ; early distal injection 97 + / - 1 vs 98 + / - 1 % , late distal injection 98 + / - 1 vs 99 + / - 1 % .
	manualset3
189763	2	415530	7	NULL	NULL	0	NULL	glucose recovery	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After distal tubular injections ( 14C ) glucose recovery was complete in both C and VE ; early distal injection 97 + / - 1 vs 98 + / - 1 % , late distal injection 98 + / - 1 vs 99 + / - 1 % .
	manualset3
189764	3	415530	7	NULL	NULL	0	NULL	C	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	After distal tubular injections ( 14C ) glucose recovery was complete in both C and VE ; early distal injection 97 + / - 1 vs 98 + / - 1 % , late distal injection 98 + / - 1 vs 99 + / - 1 % .
	manualset3
189765	4	415530	7	NULL	NULL	0	NULL	VE	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	After distal tubular injections ( 14C ) glucose recovery was complete in both C and VE ; early distal injection 97 + / - 1 vs 98 + / - 1 % , late distal injection 98 + / - 1 vs 99 + / - 1 % .
	manualset3
189766	5	415530	7	NULL	NULL	0	NULL	early distal injection 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After distal tubular injections ( 14C ) glucose recovery was complete in both C and VE ; early distal injection 97 + / - 1 vs 98 + / - 1 % , late distal injection 98 + / - 1 vs 99 + / - 1 % .
	manualset3
189767	6	415530	7	NULL	NULL	NULL	NULL	97 + / - 1 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After distal tubular injections ( 14C ) glucose recovery was complete in both C and VE ; early distal injection 97 + / - 1 vs 98 + / - 1 % , late distal injection 98 + / - 1 vs 99 + / - 1 % .
	manualset3
189768	7	415530	7	NULL	NULL	0	NULL	98 + / - 1 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	After distal tubular injections ( 14C ) glucose recovery was complete in both C and VE ; early distal injection 97 + / - 1 vs 98 + / - 1 % , late distal injection 98 + / - 1 vs 99 + / - 1 % .
	manualset3
189769	8	415530	7	NULL	NULL	0	NULL	late distal injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After distal tubular injections ( 14C ) glucose recovery was complete in both C and VE ; early distal injection 97 + / - 1 vs 98 + / - 1 % , late distal injection 98 + / - 1 vs 99 + / - 1 % .
	manualset3
189770	9	415530	7	NULL	NULL	0	NULL	98 + / - 1%	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	After distal tubular injections ( 14C ) glucose recovery was complete in both C and VE ; early distal injection 97 + / - 1 vs 98 + / - 1 % , late distal injection 98 + / - 1 vs 99 + / - 1 % .
	manualset3
189771	10	415530	7	NULL	NULL	0	NULL	99 + / - 1 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	After distal tubular injections ( 14C ) glucose recovery was complete in both C and VE ; early distal injection 97 + / - 1 vs 98 + / - 1 % , late distal injection 98 + / - 1 vs 99 + / - 1 % .
	manualset3
189775	1	415531	7	NULL	NULL	0	NULL	asymmetry	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To test whether this asymmetry generalizes across modalities , auditory ( aspirated `` pa '' and unaspirated `` ba '' stops ) and tactile ( slight , inaudible , cutaneous air puffs ) signals were presented synchronously and asynchronously .
	manualset3
189776	2	415531	7	NULL	NULL	0	NULL	modalities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To test whether this asymmetry generalizes across modalities , auditory ( aspirated `` pa '' and unaspirated `` ba '' stops ) and tactile ( slight , inaudible , cutaneous air puffs ) signals were presented synchronously and asynchronously .
	manualset3
189777	3	415531	7	NULL	NULL	0	NULL	auditory ( aspirated `` pa '' and unaspirated `` ba '' stops ) signals	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	To test whether this asymmetry generalizes across modalities , auditory ( aspirated `` pa '' and unaspirated `` ba '' stops ) and tactile ( slight , inaudible , cutaneous air puffs ) signals were presented synchronously and asynchronously .
	manualset3
189778	4	415531	7	NULL	NULL	0	NULL	tactile ( slight , inaudible , cutaneous air puffs ) signals	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	To test whether this asymmetry generalizes across modalities , auditory ( aspirated `` pa '' and unaspirated `` ba '' stops ) and tactile ( slight , inaudible , cutaneous air puffs ) signals were presented synchronously and asynchronously .
	manualset3
189781	1	415532	7	NULL	NULL	0	NULL	knowledge	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To the best of our knowledge , cribriform pedunculated adenocarcinoma of the base of the tongue has not been previously reported .
	manualset3
189782	2	415532	7	NULL	NULL	0	NULL	cribriform pedunculated adenocarcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To the best of our knowledge , cribriform pedunculated adenocarcinoma of the base of the tongue has not been previously reported .
	manualset3
189783	3	415532	7	NULL	NULL	0	NULL	base of the tongue	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To the best of our knowledge , cribriform pedunculated adenocarcinoma of the base of the tongue has not been previously reported .
	manualset3
189784	1	415533	7	NULL	NULL	0	NULL	extent	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To the extent that monkey prefrontal function can model certain aspects of human prefrontal function , we argue that this model can now be extended to the rat orbitofrontal cortex .
	manualset3
189785	2	415533	7	NULL	NULL	0	NULL	monkey prefrontal function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To the extent that monkey prefrontal function can model certain aspects of human prefrontal function , we argue that this model can now be extended to the rat orbitofrontal cortex .
	manualset3
189786	3	415533	7	NULL	NULL	0	NULL	aspects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To the extent that monkey prefrontal function can model certain aspects of human prefrontal function , we argue that this model can now be extended to the rat orbitofrontal cortex .
	manualset3
189787	4	415533	7	NULL	NULL	0	NULL	human prefrontal function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To the extent that monkey prefrontal function can model certain aspects of human prefrontal function , we argue that this model can now be extended to the rat orbitofrontal cortex .
	manualset3
189788	5	415533	7	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	To the extent that monkey prefrontal function can model certain aspects of human prefrontal function , we argue that this model can now be extended to the rat orbitofrontal cortex .
	manualset3
189789	6	415533	7	NULL	NULL	0	NULL	rat orbitofrontal cortex 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To the extent that monkey prefrontal function can model certain aspects of human prefrontal function , we argue that this model can now be extended to the rat orbitofrontal cortex .
	manualset3
189790	1	415534	7	NULL	NULL	0	NULL	processes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To this end , both processes were carried out under normal sterile conditions , using sanitized material and equipment and optimal water quality in a clean but open environment .
	manualset3
189791	2	415534	7	NULL	NULL	0	NULL	normal sterile conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	To this end , both processes were carried out under normal sterile conditions , using sanitized material and equipment and optimal water quality in a clean but open environment .
	manualset3
189792	3	415534	7	NULL	NULL	0	NULL	sanitized material	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	To this end , both processes were carried out under normal sterile conditions , using sanitized material and equipment and optimal water quality in a clean but open environment .
	manualset3
189793	4	415534	7	NULL	NULL	0	NULL	equipment	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	To this end , both processes were carried out under normal sterile conditions , using sanitized material and equipment and optimal water quality in a clean but open environment .
	manualset3
189794	5	415534	7	NULL	NULL	0	NULL	optimal water quality	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	To this end , both processes were carried out under normal sterile conditions , using sanitized material and equipment and optimal water quality in a clean but open environment .
	manualset3
189795	6	415534	7	NULL	NULL	0	NULL	open environment	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	To this end , both processes were carried out under normal sterile conditions , using sanitized material and equipment and optimal water quality in a clean but open environment .
	manualset3
189796	1	415535	7	NULL	NULL	0	NULL	semi-intensive reproductive rhythm 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To this end , does were either submitted to a semi-intensive reproductive rhythm ( Group S , inseminated on Day 11 postpartum ) or an extensive rhythm ( Group E , inseminated on Day 32 postpartum ) .
	manualset3
189797	2	415535	7	NULL	NULL	0	NULL	Group S , inseminated on Day 11 postpartum	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To this end , does were either submitted to a semi-intensive reproductive rhythm ( Group S , inseminated on Day 11 postpartum ) or an extensive rhythm ( Group E , inseminated on Day 32 postpartum ) .
	manualset3
189798	3	415535	7	NULL	NULL	0	NULL	extensive rhythm	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To this end , does were either submitted to a semi-intensive reproductive rhythm ( Group S , inseminated on Day 11 postpartum ) or an extensive rhythm ( Group E , inseminated on Day 32 postpartum ) .
	manualset3
189799	4	415535	7	NULL	NULL	0	NULL	Group E , inseminated on Day 32 postpartum 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To this end , does were either submitted to a semi-intensive reproductive rhythm ( Group S , inseminated on Day 11 postpartum ) or an extensive rhythm ( Group E , inseminated on Day 32 postpartum ) .
	manualset3
189800	1	415536	7	NULL	NULL	0	NULL	 mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To understand mechanisms of the regulation of synapse-specific transcription , we studied the promoter activity of the 5 ' - flanking region of the AChR epsilon subunit gene in response to ARIA .
	manualset3
189801	2	415536	7	NULL	NULL	0	NULL	regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To understand mechanisms of the regulation of synapse-specific transcription , we studied the promoter activity of the 5 ' - flanking region of the AChR epsilon subunit gene in response to ARIA .
	manualset3
189802	3	415536	7	NULL	NULL	0	NULL	synapse-specific transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To understand mechanisms of the regulation of synapse-specific transcription , we studied the promoter activity of the 5 ' - flanking region of the AChR epsilon subunit gene in response to ARIA .
	manualset3
189803	4	415536	7	NULL	NULL	0	NULL	promoter activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To understand mechanisms of the regulation of synapse-specific transcription , we studied the promoter activity of the 5 ' - flanking region of the AChR epsilon subunit gene in response to ARIA .
	manualset3
189804	5	415536	7	NULL	NULL	0	NULL	5 ' - flanking region	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	To understand mechanisms of the regulation of synapse-specific transcription , we studied the promoter activity of the 5 ' - flanking region of the AChR epsilon subunit gene in response to ARIA .
	manualset3
189805	6	415536	7	NULL	NULL	0	NULL	AChR epsilon subunit gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	To understand mechanisms of the regulation of synapse-specific transcription , we studied the promoter activity of the 5 ' - flanking region of the AChR epsilon subunit gene in response to ARIA .
	manualset3
189806	7	415536	7	NULL	NULL	0	NULL	response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To understand mechanisms of the regulation of synapse-specific transcription , we studied the promoter activity of the 5 ' - flanking region of the AChR epsilon subunit gene in response to ARIA .
	manualset3
189807	8	415536	7	NULL	NULL	0	NULL	ARIA	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To understand mechanisms of the regulation of synapse-specific transcription , we studied the promoter activity of the 5 ' - flanking region of the AChR epsilon subunit gene in response to ARIA .
	manualset3
189808	1	415537	7	NULL	NULL	0	NULL	significance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To understand the significance of dCyd kinase levels in chemotherapy , dCyd kinase mRNA levels were evaluated in several cells with a quantitative competitive polymerase chain reaction ( PCR ) assay .
	manualset3
189809	2	415537	7	NULL	NULL	0	NULL	dCyd kinase levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To understand the significance of dCyd kinase levels in chemotherapy , dCyd kinase mRNA levels were evaluated in several cells with a quantitative competitive polymerase chain reaction ( PCR ) assay .
	manualset3
189810	3	415537	7	NULL	NULL	0	NULL	chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To understand the significance of dCyd kinase levels in chemotherapy , dCyd kinase mRNA levels were evaluated in several cells with a quantitative competitive polymerase chain reaction ( PCR ) assay .
	manualset3
189811	4	415537	7	NULL	NULL	0	NULL	dCyd kinase mRNA levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To understand the significance of dCyd kinase levels in chemotherapy , dCyd kinase mRNA levels were evaluated in several cells with a quantitative competitive polymerase chain reaction ( PCR ) assay .
	manualset3
189812	5	415537	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To understand the significance of dCyd kinase levels in chemotherapy , dCyd kinase mRNA levels were evaluated in several cells with a quantitative competitive polymerase chain reaction ( PCR ) assay .
	manualset3
189813	6	415537	7	NULL	NULL	0	NULL	quantitative competitive polymerase chain reaction ( PCR ) assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To understand the significance of dCyd kinase levels in chemotherapy , dCyd kinase mRNA levels were evaluated in several cells with a quantitative competitive polymerase chain reaction ( PCR ) assay .
	manualset3
189814	1	415538	7	NULL	NULL	0	NULL	period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After each period of reperfusion , the rat brain was fixed by freezing in situ and used for assaying leukotrienes , vitamin A , and water content .
	manualset3
189815	2	415538	7	NULL	NULL	0	NULL	reperfusion 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After each period of reperfusion , the rat brain was fixed by freezing in situ and used for assaying leukotrienes , vitamin A , and water content .
	manualset3
189816	3	415538	7	NULL	NULL	0	NULL	rat brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After each period of reperfusion , the rat brain was fixed by freezing in situ and used for assaying leukotrienes , vitamin A , and water content .
	manualset3
189817	4	415538	7	NULL	NULL	0	NULL	freezing 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After each period of reperfusion , the rat brain was fixed by freezing in situ and used for assaying leukotrienes , vitamin A , and water content .
	manualset3
189818	5	415538	7	NULL	NULL	0	NULL	assaying	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After each period of reperfusion , the rat brain was fixed by freezing in situ and used for assaying leukotrienes , vitamin A , and water content .
	manualset3
189819	6	415538	7	NULL	NULL	0	NULL	leukotrienes	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After each period of reperfusion , the rat brain was fixed by freezing in situ and used for assaying leukotrienes , vitamin A , and water content .
	manualset3
189820	7	415538	7	NULL	NULL	0	NULL	vitamin A	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After each period of reperfusion , the rat brain was fixed by freezing in situ and used for assaying leukotrienes , vitamin A , and water content .
	manualset3
189821	8	415538	7	NULL	NULL	0	NULL	water content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After each period of reperfusion , the rat brain was fixed by freezing in situ and used for assaying leukotrienes , vitamin A , and water content .
	manualset3
189822	1	415539	7	NULL	NULL	0	NULL	 hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	To verify this hypothesis , we assessed the effect of baseball experience or skill levels on simple reaction times and Go/Nogo reaction times in 82 university students ( 22 baseball players , 22 tennis players , and 38 nonathletes ) and 17 professional baseball players .
	manualset3
189823	2	415539	7	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To verify this hypothesis , we assessed the effect of baseball experience or skill levels on simple reaction times and Go/Nogo reaction times in 82 university students ( 22 baseball players , 22 tennis players , and 38 nonathletes ) and 17 professional baseball players .
	manualset3
189824	3	415539	7	NULL	NULL	0	NULL	baseball experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To verify this hypothesis , we assessed the effect of baseball experience or skill levels on simple reaction times and Go/Nogo reaction times in 82 university students ( 22 baseball players , 22 tennis players , and 38 nonathletes ) and 17 professional baseball players .
	manualset3
189825	4	415539	7	NULL	NULL	0	NULL	skill levels	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To verify this hypothesis , we assessed the effect of baseball experience or skill levels on simple reaction times and Go/Nogo reaction times in 82 university students ( 22 baseball players , 22 tennis players , and 38 nonathletes ) and 17 professional baseball players .
	manualset3
189826	5	415539	7	NULL	NULL	0	NULL	simple reaction times	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To verify this hypothesis , we assessed the effect of baseball experience or skill levels on simple reaction times and Go/Nogo reaction times in 82 university students ( 22 baseball players , 22 tennis players , and 38 nonathletes ) and 17 professional baseball players .
	manualset3
189827	6	415539	7	NULL	NULL	0	NULL	Go/Nogo reaction times	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To verify this hypothesis , we assessed the effect of baseball experience or skill levels on simple reaction times and Go/Nogo reaction times in 82 university students ( 22 baseball players , 22 tennis players , and 38 nonathletes ) and 17 professional baseball players .
	manualset3
189828	7	415539	7	NULL	NULL	0	NULL	82 university students	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To verify this hypothesis , we assessed the effect of baseball experience or skill levels on simple reaction times and Go/Nogo reaction times in 82 university students ( 22 baseball players , 22 tennis players , and 38 nonathletes ) and 17 professional baseball players .
	manualset3
189829	8	415539	7	NULL	NULL	NULL	NULL	22 baseball players	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To verify this hypothesis , we assessed the effect of baseball experience or skill levels on simple reaction times and Go/Nogo reaction times in 82 university students ( 22 baseball players , 22 tennis players , and 38 nonathletes ) and 17 professional baseball players .
	manualset3
189830	9	415539	7	NULL	NULL	0	NULL	22 tennis players	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To verify this hypothesis , we assessed the effect of baseball experience or skill levels on simple reaction times and Go/Nogo reaction times in 82 university students ( 22 baseball players , 22 tennis players , and 38 nonathletes ) and 17 professional baseball players .
	manualset3
189831	10	415539	7	NULL	NULL	0	NULL	38 nonathletes	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To verify this hypothesis , we assessed the effect of baseball experience or skill levels on simple reaction times and Go/Nogo reaction times in 82 university students ( 22 baseball players , 22 tennis players , and 38 nonathletes ) and 17 professional baseball players .
	manualset3
189832	11	415539	7	NULL	NULL	0	NULL	17 professional baseball players	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To verify this hypothesis , we assessed the effect of baseball experience or skill levels on simple reaction times and Go/Nogo reaction times in 82 university students ( 22 baseball players , 22 tennis players , and 38 nonathletes ) and 17 professional baseball players .
	manualset3
189833	1	415540	7	NULL	NULL	0	NULL	Tobacco	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Tobacco , alcohol , asbestos , and nickel in the etiology of cancer of the larynx : a case-control study .
	manualset3
189834	2	415540	7	NULL	NULL	0	NULL	alcohol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Tobacco , alcohol , asbestos , and nickel in the etiology of cancer of the larynx : a case-control study .
	manualset3
189835	3	415540	7	NULL	NULL	0	NULL	asbestos	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Tobacco , alcohol , asbestos , and nickel in the etiology of cancer of the larynx : a case-control study .
	manualset3
189836	4	415540	7	NULL	NULL	0	NULL	 nickel	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Tobacco , alcohol , asbestos , and nickel in the etiology of cancer of the larynx : a case-control study .
	manualset3
189837	5	415540	7	NULL	NULL	0	NULL	etiology of cancer	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Tobacco , alcohol , asbestos , and nickel in the etiology of cancer of the larynx : a case-control study .
	manualset3
189838	6	415540	7	NULL	NULL	0	NULL	 larynx	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Tobacco , alcohol , asbestos , and nickel in the etiology of cancer of the larynx : a case-control study .
	manualset3
189839	7	415540	7	NULL	NULL	0	NULL	case-control study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Tobacco , alcohol , asbestos , and nickel in the etiology of cancer of the larynx : a case-control study .
	manualset3
189840	1	415541	7	NULL	NULL	0	NULL	Tobacco smoke exposure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Tobacco smoke exposure induces nicotine dependence in rats .
	manualset3
189841	2	415541	7	NULL	NULL	0	NULL	nicotine dependence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Tobacco smoke exposure induces nicotine dependence in rats .
	manualset3
189842	3	415541	7	NULL	NULL	0	NULL	 rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Tobacco smoke exposure induces nicotine dependence in rats .
	manualset3
189843	1	415542	7	NULL	NULL	0	NULL	Tobacco use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Tobacco use is high among pregnant women , but this can be a time of great motivation to begin cessation efforts .
	manualset3
189844	2	415542	7	NULL	NULL	0	NULL	pregnant women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Tobacco use is high among pregnant women , but this can be a time of great motivation to begin cessation efforts .
	manualset3
189845	3	415542	7	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Tobacco use is high among pregnant women , but this can be a time of great motivation to begin cessation efforts .
	manualset3
189846	4	415542	7	NULL	NULL	0	NULL	great motivation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Tobacco use is high among pregnant women , but this can be a time of great motivation to begin cessation efforts .
	manualset3
189847	5	415542	7	NULL	NULL	0	NULL	cessation efforts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Tobacco use is high among pregnant women , but this can be a time of great motivation to begin cessation efforts .
	manualset3
189848	1	415543	7	NULL	NULL	0	NULL	Toca-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Toca-1 or FBP17 recruited N-WASP-WIP to the membrane .
	manualset3
189849	2	415543	7	NULL	NULL	0	NULL	FBP17	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Toca-1 or FBP17 recruited N-WASP-WIP to the membrane .
	manualset3
189850	3	415543	7	NULL	NULL	0	NULL	N-WASP-WIP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Toca-1 or FBP17 recruited N-WASP-WIP to the membrane .
	manualset3
189851	4	415543	7	NULL	NULL	0	NULL	membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Toca-1 or FBP17 recruited N-WASP-WIP to the membrane .
	manualset3
189929	1	415544	7	NULL	NULL	0	NULL	HIM professional 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Today 's HIM professional can be a positive and an integral component in providing nursing clinical education .
	manualset3
189930	2	415544	7	NULL	NULL	0	NULL	 integral component 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Today 's HIM professional can be a positive and an integral component in providing nursing clinical education .
	manualset3
189931	3	415544	7	NULL	NULL	0	NULL	nursing clinical education 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Today 's HIM professional can be a positive and an integral component in providing nursing clinical education .
	manualset3
189932	1	415545	7	NULL	NULL	0	NULL	specialists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Today , however , most specialists expect to receive some form of remuneration for taking ER calls .
	manualset3
189933	2	415545	7	NULL	NULL	0	NULL	remuneration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Today , however , most specialists expect to receive some form of remuneration for taking ER calls .
	manualset3
189934	3	415545	7	NULL	NULL	0	NULL	ER calls 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Today , however , most specialists expect to receive some form of remuneration for taking ER calls .
	manualset3
189935	1	415546	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , our data suggest that Blimp-1 ensures the survival of transformed plasma cells .
	manualset3
189936	2	415546	7	NULL	NULL	0	NULL	Blimp-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , our data suggest that Blimp-1 ensures the survival of transformed plasma cells .
	manualset3
189937	3	415546	7	NULL	NULL	0	NULL	survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , our data suggest that Blimp-1 ensures the survival of transformed plasma cells .
	manualset3
189938	4	415546	7	NULL	NULL	0	NULL	transformed plasma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , our data suggest that Blimp-1 ensures the survival of transformed plasma cells .
	manualset3
189939	1	415547	7	NULL	NULL	0	NULL	observations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , our observations suggest that alpha-catenin may be a new tumor suppressor gene that operates in the E-cadherin tumor suppressor pathway .
	manualset3
189940	2	415547	7	NULL	NULL	NULL	NULL	alpha-catenin	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Together , our observations suggest that alpha-catenin may be a new tumor suppressor gene that operates in the E-cadherin tumor suppressor pathway .
	manualset3
189941	3	415547	7	NULL	NULL	0	NULL	tumor suppressor gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , our observations suggest that alpha-catenin may be a new tumor suppressor gene that operates in the E-cadherin tumor suppressor pathway .
	manualset3
189942	4	415547	7	NULL	NULL	0	NULL	 E-cadherin tumor suppressor pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , our observations suggest that alpha-catenin may be a new tumor suppressor gene that operates in the E-cadherin tumor suppressor pathway .
	manualset3
189943	1	415548	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , our results suggest that the aberrant activation of the ISG15 pathway confers a motile phenotype to breast cancer cells by disrupting cell architecture and stabilizing proteins involved in cell motility , invasion and metastasis .
	manualset3
189944	2	415548	7	NULL	NULL	0	NULL	aberrant activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , our results suggest that the aberrant activation of the ISG15 pathway confers a motile phenotype to breast cancer cells by disrupting cell architecture and stabilizing proteins involved in cell motility , invasion and metastasis .
	manualset3
189945	3	415548	7	NULL	NULL	0	NULL	ISG15 pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , our results suggest that the aberrant activation of the ISG15 pathway confers a motile phenotype to breast cancer cells by disrupting cell architecture and stabilizing proteins involved in cell motility , invasion and metastasis .
	manualset3
189946	4	415548	7	NULL	NULL	0	NULL	motile phenotype	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , our results suggest that the aberrant activation of the ISG15 pathway confers a motile phenotype to breast cancer cells by disrupting cell architecture and stabilizing proteins involved in cell motility , invasion and metastasis .
	manualset3
189947	5	415548	7	NULL	NULL	0	NULL	 breast cancer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , our results suggest that the aberrant activation of the ISG15 pathway confers a motile phenotype to breast cancer cells by disrupting cell architecture and stabilizing proteins involved in cell motility , invasion and metastasis .
	manualset3
189948	6	415548	7	NULL	NULL	0	NULL	cell architecture	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , our results suggest that the aberrant activation of the ISG15 pathway confers a motile phenotype to breast cancer cells by disrupting cell architecture and stabilizing proteins involved in cell motility , invasion and metastasis .
	manualset3
189949	7	415548	7	NULL	NULL	0	NULL	proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , our results suggest that the aberrant activation of the ISG15 pathway confers a motile phenotype to breast cancer cells by disrupting cell architecture and stabilizing proteins involved in cell motility , invasion and metastasis .
	manualset3
189950	8	415548	7	NULL	NULL	0	NULL	cell motility	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , our results suggest that the aberrant activation of the ISG15 pathway confers a motile phenotype to breast cancer cells by disrupting cell architecture and stabilizing proteins involved in cell motility , invasion and metastasis .
	manualset3
189951	9	415548	7	NULL	NULL	0	NULL	invasion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , our results suggest that the aberrant activation of the ISG15 pathway confers a motile phenotype to breast cancer cells by disrupting cell architecture and stabilizing proteins involved in cell motility , invasion and metastasis .
	manualset3
189952	10	415548	7	NULL	NULL	0	NULL	metastasis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , our results suggest that the aberrant activation of the ISG15 pathway confers a motile phenotype to breast cancer cells by disrupting cell architecture and stabilizing proteins involved in cell motility , invasion and metastasis .
	manualset3
189953	1	415549	7	NULL	NULL	0	NULL	TIAF1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , TIAF1 shows an aggregation-dependent control of tumor progression and metastasis , and regulation of cell death .
	manualset3
189954	2	415549	7	NULL	NULL	0	NULL	aggregation-dependent control	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , TIAF1 shows an aggregation-dependent control of tumor progression and metastasis , and regulation of cell death .
	manualset3
189955	3	415549	7	NULL	NULL	0	NULL	tumor progression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , TIAF1 shows an aggregation-dependent control of tumor progression and metastasis , and regulation of cell death .
	manualset3
189956	4	415549	7	NULL	NULL	0	NULL	metastasis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , TIAF1 shows an aggregation-dependent control of tumor progression and metastasis , and regulation of cell death .
	manualset3
189957	5	415549	7	NULL	NULL	0	NULL	 regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , TIAF1 shows an aggregation-dependent control of tumor progression and metastasis , and regulation of cell death .
	manualset3
189958	6	415549	7	NULL	NULL	NULL	NULL	cell death	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Together , TIAF1 shows an aggregation-dependent control of tumor progression and metastasis , and regulation of cell death .
	manualset3
189959	1	415550	7	NULL	NULL	0	NULL	entry	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After entry the vast majority of heterologous DNA was found at the single-strand DNA position in CsCl gradients , and was gradually degraded during incubation .
	manualset3
189960	2	415550	7	NULL	NULL	0	NULL	vast majority 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After entry the vast majority of heterologous DNA was found at the single-strand DNA position in CsCl gradients , and was gradually degraded during incubation .
	manualset3
189961	3	415550	7	NULL	NULL	0	NULL	heterologous DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	After entry the vast majority of heterologous DNA was found at the single-strand DNA position in CsCl gradients , and was gradually degraded during incubation .
	manualset3
189962	4	415550	7	NULL	NULL	0	NULL	single-strand DNA position	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	After entry the vast majority of heterologous DNA was found at the single-strand DNA position in CsCl gradients , and was gradually degraded during incubation .
	manualset3
189963	5	415550	7	NULL	NULL	0	NULL	CsCl gradients	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After entry the vast majority of heterologous DNA was found at the single-strand DNA position in CsCl gradients , and was gradually degraded during incubation .
	manualset3
189964	6	415550	7	NULL	NULL	0	NULL	incubation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After entry the vast majority of heterologous DNA was found at the single-strand DNA position in CsCl gradients , and was gradually degraded during incubation .
	manualset3
189965	1	415551	7	NULL	NULL	0	NULL	 new information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , the new information gained about the vitamin K-dependent gamma-carboxylation system will stimulate new research which will benefit medicine and our understanding of the molecular mechanisms involved in this protein modification reaction .
	manualset3
189966	2	415551	7	NULL	NULL	0	NULL	vitamin K-dependent gamma-carboxylation system	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , the new information gained about the vitamin K-dependent gamma-carboxylation system will stimulate new research which will benefit medicine and our understanding of the molecular mechanisms involved in this protein modification reaction .
	manualset3
189967	3	415551	7	NULL	NULL	0	NULL	new research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , the new information gained about the vitamin K-dependent gamma-carboxylation system will stimulate new research which will benefit medicine and our understanding of the molecular mechanisms involved in this protein modification reaction .
	manualset3
189968	4	415551	7	NULL	NULL	0	NULL	medicine	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , the new information gained about the vitamin K-dependent gamma-carboxylation system will stimulate new research which will benefit medicine and our understanding of the molecular mechanisms involved in this protein modification reaction .
	manualset3
189969	5	415551	7	NULL	NULL	0	NULL	understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , the new information gained about the vitamin K-dependent gamma-carboxylation system will stimulate new research which will benefit medicine and our understanding of the molecular mechanisms involved in this protein modification reaction .
	manualset3
189970	6	415551	7	NULL	NULL	0	NULL	molecular mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , the new information gained about the vitamin K-dependent gamma-carboxylation system will stimulate new research which will benefit medicine and our understanding of the molecular mechanisms involved in this protein modification reaction .
	manualset3
189971	7	415551	7	NULL	NULL	0	NULL	protein modification reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , the new information gained about the vitamin K-dependent gamma-carboxylation system will stimulate new research which will benefit medicine and our understanding of the molecular mechanisms involved in this protein modification reaction .
	manualset3
189976	1	415552	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these data suggest that , unlike many other G protein-coupled receptors , FPR does not form homodimers .
	manualset3
189979	2	415552	7	NULL	NULL	0	NULL	G protein-coupled receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these data suggest that , unlike many other G protein-coupled receptors , FPR does not form homodimers .
	manualset3
189980	3	415552	7	NULL	NULL	0	NULL	FPR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these data suggest that , unlike many other G protein-coupled receptors , FPR does not form homodimers .
	manualset3
189983	4	415552	7	NULL	NULL	0	NULL	homodimers	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these data suggest that , unlike many other G protein-coupled receptors , FPR does not form homodimers .
	manualset3
189985	1	415553	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these data suggest that POSH has a distinct role as a specific E3 ubiquitin ligase for Hrs on early endosomes , and there exists a relationship between its separate activities as a scaffold and as an E3 .
	manualset3
189986	2	415553	7	NULL	NULL	0	NULL	POSH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these data suggest that POSH has a distinct role as a specific E3 ubiquitin ligase for Hrs on early endosomes , and there exists a relationship between its separate activities as a scaffold and as an E3 .
	manualset3
189987	3	415553	7	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these data suggest that POSH has a distinct role as a specific E3 ubiquitin ligase for Hrs on early endosomes , and there exists a relationship between its separate activities as a scaffold and as an E3 .
	manualset3
189988	4	415553	7	NULL	NULL	0	NULL	E3 ubiquitin ligase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these data suggest that POSH has a distinct role as a specific E3 ubiquitin ligase for Hrs on early endosomes , and there exists a relationship between its separate activities as a scaffold and as an E3 .
	manualset3
189989	5	415553	7	NULL	NULL	0	NULL	Hrs 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these data suggest that POSH has a distinct role as a specific E3 ubiquitin ligase for Hrs on early endosomes , and there exists a relationship between its separate activities as a scaffold and as an E3 .
	manualset3
189990	6	415553	7	NULL	NULL	0	NULL	early endosomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these data suggest that POSH has a distinct role as a specific E3 ubiquitin ligase for Hrs on early endosomes , and there exists a relationship between its separate activities as a scaffold and as an E3 .
	manualset3
189991	7	415553	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these data suggest that POSH has a distinct role as a specific E3 ubiquitin ligase for Hrs on early endosomes , and there exists a relationship between its separate activities as a scaffold and as an E3 .
	manualset3
189992	8	415553	7	NULL	NULL	0	NULL	activities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these data suggest that POSH has a distinct role as a specific E3 ubiquitin ligase for Hrs on early endosomes , and there exists a relationship between its separate activities as a scaffold and as an E3 .
	manualset3
189993	9	415553	7	NULL	NULL	0	NULL	scaffold	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these data suggest that POSH has a distinct role as a specific E3 ubiquitin ligase for Hrs on early endosomes , and there exists a relationship between its separate activities as a scaffold and as an E3 .
	manualset3
189994	10	415553	7	NULL	NULL	0	NULL	E3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these data suggest that POSH has a distinct role as a specific E3 ubiquitin ligase for Hrs on early endosomes , and there exists a relationship between its separate activities as a scaffold and as an E3 .
	manualset3
190077	1	415554	7	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these data suggest that ribosomal changes resulting from cold shock may be responsible for the decrease in D value observed when L. monocytogenes is cold shocked .
	manualset3
190078	2	415554	7	NULL	NULL	0	NULL	ribosomal changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these data suggest that ribosomal changes resulting from cold shock may be responsible for the decrease in D value observed when L. monocytogenes is cold shocked .
	manualset3
190079	3	415554	7	NULL	NULL	0	NULL	cold shock	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these data suggest that ribosomal changes resulting from cold shock may be responsible for the decrease in D value observed when L. monocytogenes is cold shocked .
	manualset3
190081	4	415554	7	NULL	NULL	0	NULL	decrease	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these data suggest that ribosomal changes resulting from cold shock may be responsible for the decrease in D value observed when L. monocytogenes is cold shocked .
	manualset3
190082	5	415554	7	NULL	NULL	0	NULL	D value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these data suggest that ribosomal changes resulting from cold shock may be responsible for the decrease in D value observed when L. monocytogenes is cold shocked .
	manualset3
190084	6	415554	7	NULL	NULL	0	NULL	L. monocytogenes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these data suggest that ribosomal changes resulting from cold shock may be responsible for the decrease in D value observed when L. monocytogenes is cold shocked .
	manualset3
190089	1	415555	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these findings suggest that multi-layered , microfabricated PGS scaffolds may be applicable to myocardial repair applications requiring mechanical support , cell delivery and active implant contractility .
	manualset3
190092	2	415555	7	NULL	NULL	0	NULL	multi-layered , microfabricated PGS scaffolds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these findings suggest that multi-layered , microfabricated PGS scaffolds may be applicable to myocardial repair applications requiring mechanical support , cell delivery and active implant contractility .
	manualset3
190110	3	415555	7	NULL	NULL	0	NULL	myocardial repair applications	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these findings suggest that multi-layered , microfabricated PGS scaffolds may be applicable to myocardial repair applications requiring mechanical support , cell delivery and active implant contractility .
	manualset3
190112	4	415555	7	NULL	NULL	0	NULL	mechanical support	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these findings suggest that multi-layered , microfabricated PGS scaffolds may be applicable to myocardial repair applications requiring mechanical support , cell delivery and active implant contractility .
	manualset3
190113	5	415555	7	NULL	NULL	0	NULL	cell delivery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these findings suggest that multi-layered , microfabricated PGS scaffolds may be applicable to myocardial repair applications requiring mechanical support , cell delivery and active implant contractility .
	manualset3
190114	6	415555	7	NULL	NULL	0	NULL	active implant contractility	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these findings suggest that multi-layered , microfabricated PGS scaffolds may be applicable to myocardial repair applications requiring mechanical support , cell delivery and active implant contractility .
	manualset3
190122	1	415556	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these results highlight the potential for pro-resolving mediators in prolonging survival of solid organ transplants .
	manualset3
190126	2	415556	7	NULL	NULL	0	NULL	pro-resolving mediators	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these results highlight the potential for pro-resolving mediators in prolonging survival of solid organ transplants .
	manualset3
190127	3	415556	7	NULL	NULL	0	NULL	prolonging survival 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these results highlight the potential for pro-resolving mediators in prolonging survival of solid organ transplants .
	manualset3
190128	4	415556	7	NULL	NULL	0	NULL	solid organ transplants	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these results highlight the potential for pro-resolving mediators in prolonging survival of solid organ transplants .
	manualset3
190129	1	415557	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these results indicate that MMP-2 may be primarily associated with the development and differentiation of cortical plate neurons and wound recovery processes .
	manualset3
190130	2	415557	7	NULL	NULL	0	NULL	MMP-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these results indicate that MMP-2 may be primarily associated with the development and differentiation of cortical plate neurons and wound recovery processes .
	manualset3
190131	3	415557	7	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these results indicate that MMP-2 may be primarily associated with the development and differentiation of cortical plate neurons and wound recovery processes .
	manualset3
190132	4	415557	7	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these results indicate that MMP-2 may be primarily associated with the development and differentiation of cortical plate neurons and wound recovery processes .
	manualset3
190134	5	415557	7	NULL	NULL	0	NULL	cortical plate neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these results indicate that MMP-2 may be primarily associated with the development and differentiation of cortical plate neurons and wound recovery processes .
	manualset3
190135	6	415557	7	NULL	NULL	0	NULL	wound recovery processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these results indicate that MMP-2 may be primarily associated with the development and differentiation of cortical plate neurons and wound recovery processes .
	manualset3
190138	1	415558	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these results suggest that EWS/FLI1 induces both DBD-dependent and DBD-independent oncogenic pathways .
	manualset3
190143	2	415558	7	NULL	NULL	0	NULL	EWS/FLI1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these results suggest that EWS/FLI1 induces both DBD-dependent and DBD-independent oncogenic pathways .
	manualset3
190144	3	415558	7	NULL	NULL	0	NULL	DBD-dependent oncogenic pathways 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these results suggest that EWS/FLI1 induces both DBD-dependent and DBD-independent oncogenic pathways .
	manualset3
190146	4	415558	7	NULL	NULL	0	NULL	DBD-independent oncogenic pathways	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Together , these results suggest that EWS/FLI1 induces both DBD-dependent and DBD-independent oncogenic pathways .
	manualset3
190154	1	415559	7	NULL	NULL	0	NULL	finding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Together with the finding that PMS-1077-treated HL-60 cells exhibited activities of differentiation by examining their ability of phagocytosing latex beads , an antiproliferative effect and a differentiation-inducing role were determined for PMS-1077 in HL-60 cells .
	manualset3
190155	2	415559	7	NULL	NULL	0	NULL	PMS-1077-treated HL-60 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Together with the finding that PMS-1077-treated HL-60 cells exhibited activities of differentiation by examining their ability of phagocytosing latex beads , an antiproliferative effect and a differentiation-inducing role were determined for PMS-1077 in HL-60 cells .
	manualset3
190157	3	415559	7	NULL	NULL	0	NULL	activities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Together with the finding that PMS-1077-treated HL-60 cells exhibited activities of differentiation by examining their ability of phagocytosing latex beads , an antiproliferative effect and a differentiation-inducing role were determined for PMS-1077 in HL-60 cells .
	manualset3
190159	4	415559	7	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Together with the finding that PMS-1077-treated HL-60 cells exhibited activities of differentiation by examining their ability of phagocytosing latex beads , an antiproliferative effect and a differentiation-inducing role were determined for PMS-1077 in HL-60 cells .
	manualset3
190161	5	415559	7	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Together with the finding that PMS-1077-treated HL-60 cells exhibited activities of differentiation by examining their ability of phagocytosing latex beads , an antiproliferative effect and a differentiation-inducing role were determined for PMS-1077 in HL-60 cells .
	manualset3
190163	6	415559	7	NULL	NULL	0	NULL	phagocytosing latex beads	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Together with the finding that PMS-1077-treated HL-60 cells exhibited activities of differentiation by examining their ability of phagocytosing latex beads , an antiproliferative effect and a differentiation-inducing role were determined for PMS-1077 in HL-60 cells .
	manualset3
190164	7	415559	7	NULL	NULL	0	NULL	antiproliferative effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Together with the finding that PMS-1077-treated HL-60 cells exhibited activities of differentiation by examining their ability of phagocytosing latex beads , an antiproliferative effect and a differentiation-inducing role were determined for PMS-1077 in HL-60 cells .
	manualset3
190165	8	415559	7	NULL	NULL	0	NULL	differentiation-inducing role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Together with the finding that PMS-1077-treated HL-60 cells exhibited activities of differentiation by examining their ability of phagocytosing latex beads , an antiproliferative effect and a differentiation-inducing role were determined for PMS-1077 in HL-60 cells .
	manualset3
190166	9	415559	7	NULL	NULL	0	NULL	PMS-1077	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Together with the finding that PMS-1077-treated HL-60 cells exhibited activities of differentiation by examining their ability of phagocytosing latex beads , an antiproliferative effect and a differentiation-inducing role were determined for PMS-1077 in HL-60 cells .
	manualset3
190168	10	415559	7	NULL	NULL	0	NULL	HL-60 cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Together with the finding that PMS-1077-treated HL-60 cells exhibited activities of differentiation by examining their ability of phagocytosing latex beads , an antiproliferative effect and a differentiation-inducing role were determined for PMS-1077 in HL-60 cells .
	manualset3
190171	1	415560	7	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After exposure for 2 days , expression levels of amelogenin and enamelin strongly increased in response to the silica-based components , while no significant change was seen for ameloblastin .
	manualset3
190174	2	415560	7	NULL	NULL	0	NULL	2 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After exposure for 2 days , expression levels of amelogenin and enamelin strongly increased in response to the silica-based components , while no significant change was seen for ameloblastin .
	manualset3
190176	3	415560	7	NULL	NULL	0	NULL	expression levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After exposure for 2 days , expression levels of amelogenin and enamelin strongly increased in response to the silica-based components , while no significant change was seen for ameloblastin .
	manualset3
190180	4	415560	7	NULL	NULL	0	NULL	amelogenin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	After exposure for 2 days , expression levels of amelogenin and enamelin strongly increased in response to the silica-based components , while no significant change was seen for ameloblastin .
	manualset3
190181	5	415560	7	NULL	NULL	0	NULL	enamelin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	After exposure for 2 days , expression levels of amelogenin and enamelin strongly increased in response to the silica-based components , while no significant change was seen for ameloblastin .
	manualset3
190182	6	415560	7	NULL	NULL	0	NULL	silica-based components	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After exposure for 2 days , expression levels of amelogenin and enamelin strongly increased in response to the silica-based components , while no significant change was seen for ameloblastin .
	manualset3
190185	7	415560	7	NULL	NULL	0	NULL	no significant change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After exposure for 2 days , expression levels of amelogenin and enamelin strongly increased in response to the silica-based components , while no significant change was seen for ameloblastin .
	manualset3
190188	8	415560	7	NULL	NULL	0	NULL	ameloblastin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	After exposure for 2 days , expression levels of amelogenin and enamelin strongly increased in response to the silica-based components , while no significant change was seen for ameloblastin .
	manualset3
190250	1	415561	7	NULL	NULL	NULL	NULL	Tolbutamide	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Tolbutamide ( 100 microM ) was found to induce no effect or to elicit a small depolarization of obese rat GR neurones in the absence of glucose , in contrast to its clear excitatory actions on control or lean Zucker GR neurones .
	manualset3
190251	2	415561	7	NULL	NULL	0	NULL	100 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Tolbutamide ( 100 microM ) was found to induce no effect or to elicit a small depolarization of obese rat GR neurones in the absence of glucose , in contrast to its clear excitatory actions on control or lean Zucker GR neurones .
	manualset3
190252	3	415561	7	NULL	NULL	0	NULL	no effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Tolbutamide ( 100 microM ) was found to induce no effect or to elicit a small depolarization of obese rat GR neurones in the absence of glucose , in contrast to its clear excitatory actions on control or lean Zucker GR neurones .
	manualset3
190253	4	415561	7	NULL	NULL	0	NULL	small depolarization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Tolbutamide ( 100 microM ) was found to induce no effect or to elicit a small depolarization of obese rat GR neurones in the absence of glucose , in contrast to its clear excitatory actions on control or lean Zucker GR neurones .
	manualset3
190255	5	415561	7	NULL	NULL	0	NULL	obese rat GR neurones	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Tolbutamide ( 100 microM ) was found to induce no effect or to elicit a small depolarization of obese rat GR neurones in the absence of glucose , in contrast to its clear excitatory actions on control or lean Zucker GR neurones .
	manualset3
190258	6	415561	7	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Tolbutamide ( 100 microM ) was found to induce no effect or to elicit a small depolarization of obese rat GR neurones in the absence of glucose , in contrast to its clear excitatory actions on control or lean Zucker GR neurones .
	manualset3
190260	7	415561	7	NULL	NULL	0	NULL	glucose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Tolbutamide ( 100 microM ) was found to induce no effect or to elicit a small depolarization of obese rat GR neurones in the absence of glucose , in contrast to its clear excitatory actions on control or lean Zucker GR neurones .
	manualset3
190261	8	415561	7	NULL	NULL	0	NULL	excitatory actions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Tolbutamide ( 100 microM ) was found to induce no effect or to elicit a small depolarization of obese rat GR neurones in the absence of glucose , in contrast to its clear excitatory actions on control or lean Zucker GR neurones .
	manualset3
190262	9	415561	7	NULL	NULL	0	NULL	control GR neurones	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Tolbutamide ( 100 microM ) was found to induce no effect or to elicit a small depolarization of obese rat GR neurones in the absence of glucose , in contrast to its clear excitatory actions on control or lean Zucker GR neurones .
	manualset3
190263	10	415561	7	NULL	NULL	0	NULL	lean Zucker GR neurones	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Tolbutamide ( 100 microM ) was found to induce no effect or to elicit a small depolarization of obese rat GR neurones in the absence of glucose , in contrast to its clear excitatory actions on control or lean Zucker GR neurones .
	manualset3
190272	1	415562	7	NULL	NULL	0	NULL	Tolerance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Tolerance to anesthesia depends on synaptic proteins .
	manualset3
190273	2	415562	7	NULL	NULL	NULL	NULL	anesthesia	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Tolerance to anesthesia depends on synaptic proteins .
	manualset3
190276	3	415562	7	NULL	NULL	NULL	NULL	synaptic proteins 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Tolerance to anesthesia depends on synaptic proteins .
	manualset3
190279	1	415563	7	NULL	NULL	0	NULL	Tolerance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Tolerance , cross-tolerance , and dependence in chronic alcoholics may in part result from membrane alterations that inhibit the binding of ethanol and other drugs .
	manualset3
190280	2	415563	7	NULL	NULL	0	NULL	cross-tolerance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Tolerance , cross-tolerance , and dependence in chronic alcoholics may in part result from membrane alterations that inhibit the binding of ethanol and other drugs .
	manualset3
190281	3	415563	7	NULL	NULL	0	NULL	dependence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Tolerance , cross-tolerance , and dependence in chronic alcoholics may in part result from membrane alterations that inhibit the binding of ethanol and other drugs .
	manualset3
190282	4	415563	7	NULL	NULL	0	NULL	chronic alcoholics	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Tolerance , cross-tolerance , and dependence in chronic alcoholics may in part result from membrane alterations that inhibit the binding of ethanol and other drugs .
	manualset3
190283	5	415563	7	NULL	NULL	0	NULL	membrane alterations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Tolerance , cross-tolerance , and dependence in chronic alcoholics may in part result from membrane alterations that inhibit the binding of ethanol and other drugs .
	manualset3
190284	6	415563	7	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Tolerance , cross-tolerance , and dependence in chronic alcoholics may in part result from membrane alterations that inhibit the binding of ethanol and other drugs .
	manualset3
190285	7	415563	7	NULL	NULL	0	NULL	ethanol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Tolerance , cross-tolerance , and dependence in chronic alcoholics may in part result from membrane alterations that inhibit the binding of ethanol and other drugs .
	manualset3
190286	8	415563	7	NULL	NULL	0	NULL	drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Tolerance , cross-tolerance , and dependence in chronic alcoholics may in part result from membrane alterations that inhibit the binding of ethanol and other drugs .
	manualset3
190320	1	415564	7	NULL	NULL	0	NULL	Tolerance induction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Tolerance induction by CTB was dose and time dependent .
	manualset3
190327	2	415564	7	NULL	NULL	0	NULL	CTB	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Tolerance induction by CTB was dose and time dependent .
	manualset3
190339	3	415564	7	NULL	NULL	0	NULL	 dose dependent	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Tolerance induction by CTB was dose and time dependent .
	manualset3
190340	4	415564	7	NULL	NULL	0	NULL	time dependent	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Tolerance induction by CTB was dose and time dependent .
	manualset3
190341	1	415565	7	NULL	NULL	0	NULL	Tolerance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Tolerance of ruminant animals to high dose in-feed administration of a selenium-enriched yeast .
	manualset3
190342	2	415565	7	NULL	NULL	0	NULL	ruminant animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Tolerance of ruminant animals to high dose in-feed administration of a selenium-enriched yeast .
	manualset3
190343	3	415565	7	NULL	NULL	0	NULL	high dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Tolerance of ruminant animals to high dose in-feed administration of a selenium-enriched yeast .
	manualset3
190344	4	415565	7	NULL	NULL	0	NULL	 in-feed administration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Tolerance of ruminant animals to high dose in-feed administration of a selenium-enriched yeast .
	manualset3
190345	5	415565	7	NULL	NULL	0	NULL	selenium-enriched yeast	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Tolerance of ruminant animals to high dose in-feed administration of a selenium-enriched yeast .
	manualset3
190346	1	415566	7	NULL	NULL	0	NULL	Toll-like receptors ( TLRs )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Toll-like receptors ( TLRs ) play critical roles in bridging the innate and adaptive immune responses .
	manualset3
190347	2	415566	7	NULL	NULL	0	NULL	critical roles	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Toll-like receptors ( TLRs ) play critical roles in bridging the innate and adaptive immune responses .
	manualset3
190348	3	415566	7	NULL	NULL	0	NULL	innate immune responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Toll-like receptors ( TLRs ) play critical roles in bridging the innate and adaptive immune responses .
	manualset3
190349	4	415566	7	NULL	NULL	0	NULL	adaptive immune responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Toll-like receptors ( TLRs ) play critical roles in bridging the innate and adaptive immune responses .
	manualset3
190350	1	415567	7	NULL	NULL	0	NULL	extensive analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After extensive analysis , no demographic group was shown to have a significantly greater risk of suicide and no geographical area had significantly higher rates than another .
	manualset3
190351	2	415567	7	NULL	NULL	0	NULL	no demographic group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	After extensive analysis , no demographic group was shown to have a significantly greater risk of suicide and no geographical area had significantly higher rates than another .
	manualset3
190352	3	415567	7	NULL	NULL	0	NULL	greater risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After extensive analysis , no demographic group was shown to have a significantly greater risk of suicide and no geographical area had significantly higher rates than another .
	manualset3
190353	4	415567	7	NULL	NULL	0	NULL	suicide 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After extensive analysis , no demographic group was shown to have a significantly greater risk of suicide and no geographical area had significantly higher rates than another .
	manualset3
190354	5	415567	7	NULL	NULL	0	NULL	no geographical area	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	After extensive analysis , no demographic group was shown to have a significantly greater risk of suicide and no geographical area had significantly higher rates than another .
	manualset3
190355	6	415567	7	NULL	NULL	0	NULL	higher rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After extensive analysis , no demographic group was shown to have a significantly greater risk of suicide and no geographical area had significantly higher rates than another .
	manualset3
190356	1	415568	7	NULL	NULL	0	NULL	ganciclovir	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical ganciclovir in the treatment of acute herpetic keratitis .
	manualset3
190357	2	415568	7	NULL	NULL	0	NULL	 treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical ganciclovir in the treatment of acute herpetic keratitis .
	manualset3
190358	3	415568	7	NULL	NULL	0	NULL	acute herpetic keratitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical ganciclovir in the treatment of acute herpetic keratitis .
	manualset3
190359	1	415569	7	NULL	NULL	0	NULL	Topical therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical therapy is the mainstay of dermatologic management of acute or localized itch or in patients with contraindications to systemic therapies .
	manualset3
190360	2	415569	7	NULL	NULL	0	NULL	dermatologic management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical therapy is the mainstay of dermatologic management of acute or localized itch or in patients with contraindications to systemic therapies .
	manualset3
190361	3	415569	7	NULL	NULL	0	NULL	acute or localized itch	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical therapy is the mainstay of dermatologic management of acute or localized itch or in patients with contraindications to systemic therapies .
	manualset3
190362	4	415569	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical therapy is the mainstay of dermatologic management of acute or localized itch or in patients with contraindications to systemic therapies .
	manualset3
190363	5	415569	7	NULL	NULL	0	NULL	contraindications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical therapy is the mainstay of dermatologic management of acute or localized itch or in patients with contraindications to systemic therapies .
	manualset3
190364	6	415569	7	NULL	NULL	0	NULL	systemic therapies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical therapy is the mainstay of dermatologic management of acute or localized itch or in patients with contraindications to systemic therapies .
	manualset3
193042	7	415569	7	NULL	NULL	0	NULL	mainstay	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical therapy is the mainstay of dermatologic management of acute or localized itch or in patients with contraindications to systemic therapies .
	manualset3
190365	1	415570	7	NULL	NULL	0	NULL	Topical treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical treatment of skin with all-trans-retinoic acid ( ATRA ) , the major biologically active form of vitamin A , results in hyperproliferation of basal keratinocytes , leading to an accelerated turnover of epidermis cells and thickening of the epidermis , probably via induction of production of paracrine growth factors for keratinocytes in epidermal suprabasal keratinocytes and/or dermal fibroblasts .
	manualset3
190366	2	415570	7	NULL	NULL	0	NULL	skin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical treatment of skin with all-trans-retinoic acid ( ATRA ) , the major biologically active form of vitamin A , results in hyperproliferation of basal keratinocytes , leading to an accelerated turnover of epidermis cells and thickening of the epidermis , probably via induction of production of paracrine growth factors for keratinocytes in epidermal suprabasal keratinocytes and/or dermal fibroblasts .
	manualset3
190367	3	415570	7	NULL	NULL	0	NULL	all-trans-retinoic acid ( ATRA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical treatment of skin with all-trans-retinoic acid ( ATRA ) , the major biologically active form of vitamin A , results in hyperproliferation of basal keratinocytes , leading to an accelerated turnover of epidermis cells and thickening of the epidermis , probably via induction of production of paracrine growth factors for keratinocytes in epidermal suprabasal keratinocytes and/or dermal fibroblasts .
	manualset3
190368	4	415570	7	NULL	NULL	0	NULL	major biologically active form	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical treatment of skin with all-trans-retinoic acid ( ATRA ) , the major biologically active form of vitamin A , results in hyperproliferation of basal keratinocytes , leading to an accelerated turnover of epidermis cells and thickening of the epidermis , probably via induction of production of paracrine growth factors for keratinocytes in epidermal suprabasal keratinocytes and/or dermal fibroblasts .
	manualset3
190369	5	415570	7	NULL	NULL	0	NULL	vitamin A	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical treatment of skin with all-trans-retinoic acid ( ATRA ) , the major biologically active form of vitamin A , results in hyperproliferation of basal keratinocytes , leading to an accelerated turnover of epidermis cells and thickening of the epidermis , probably via induction of production of paracrine growth factors for keratinocytes in epidermal suprabasal keratinocytes and/or dermal fibroblasts .
	manualset3
190370	6	415570	7	NULL	NULL	0	NULL	hyperproliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical treatment of skin with all-trans-retinoic acid ( ATRA ) , the major biologically active form of vitamin A , results in hyperproliferation of basal keratinocytes , leading to an accelerated turnover of epidermis cells and thickening of the epidermis , probably via induction of production of paracrine growth factors for keratinocytes in epidermal suprabasal keratinocytes and/or dermal fibroblasts .
	manualset3
190371	7	415570	7	NULL	NULL	0	NULL	basal keratinocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical treatment of skin with all-trans-retinoic acid ( ATRA ) , the major biologically active form of vitamin A , results in hyperproliferation of basal keratinocytes , leading to an accelerated turnover of epidermis cells and thickening of the epidermis , probably via induction of production of paracrine growth factors for keratinocytes in epidermal suprabasal keratinocytes and/or dermal fibroblasts .
	manualset3
190372	8	415570	7	NULL	NULL	0	NULL	accelerated turnover	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical treatment of skin with all-trans-retinoic acid ( ATRA ) , the major biologically active form of vitamin A , results in hyperproliferation of basal keratinocytes , leading to an accelerated turnover of epidermis cells and thickening of the epidermis , probably via induction of production of paracrine growth factors for keratinocytes in epidermal suprabasal keratinocytes and/or dermal fibroblasts .
	manualset3
190373	9	415570	7	NULL	NULL	0	NULL	epidermis cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical treatment of skin with all-trans-retinoic acid ( ATRA ) , the major biologically active form of vitamin A , results in hyperproliferation of basal keratinocytes , leading to an accelerated turnover of epidermis cells and thickening of the epidermis , probably via induction of production of paracrine growth factors for keratinocytes in epidermal suprabasal keratinocytes and/or dermal fibroblasts .
	manualset3
190374	10	415570	7	NULL	NULL	0	NULL	thickening	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical treatment of skin with all-trans-retinoic acid ( ATRA ) , the major biologically active form of vitamin A , results in hyperproliferation of basal keratinocytes , leading to an accelerated turnover of epidermis cells and thickening of the epidermis , probably via induction of production of paracrine growth factors for keratinocytes in epidermal suprabasal keratinocytes and/or dermal fibroblasts .
	manualset3
190375	11	415570	7	NULL	NULL	0	NULL	epidermis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical treatment of skin with all-trans-retinoic acid ( ATRA ) , the major biologically active form of vitamin A , results in hyperproliferation of basal keratinocytes , leading to an accelerated turnover of epidermis cells and thickening of the epidermis , probably via induction of production of paracrine growth factors for keratinocytes in epidermal suprabasal keratinocytes and/or dermal fibroblasts .
	manualset3
190376	12	415570	7	NULL	NULL	0	NULL	 induction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical treatment of skin with all-trans-retinoic acid ( ATRA ) , the major biologically active form of vitamin A , results in hyperproliferation of basal keratinocytes , leading to an accelerated turnover of epidermis cells and thickening of the epidermis , probably via induction of production of paracrine growth factors for keratinocytes in epidermal suprabasal keratinocytes and/or dermal fibroblasts .
	manualset3
190377	13	415570	7	NULL	NULL	0	NULL	production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical treatment of skin with all-trans-retinoic acid ( ATRA ) , the major biologically active form of vitamin A , results in hyperproliferation of basal keratinocytes , leading to an accelerated turnover of epidermis cells and thickening of the epidermis , probably via induction of production of paracrine growth factors for keratinocytes in epidermal suprabasal keratinocytes and/or dermal fibroblasts .
	manualset3
190378	14	415570	7	NULL	NULL	0	NULL	paracrine growth factors	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical treatment of skin with all-trans-retinoic acid ( ATRA ) , the major biologically active form of vitamin A , results in hyperproliferation of basal keratinocytes , leading to an accelerated turnover of epidermis cells and thickening of the epidermis , probably via induction of production of paracrine growth factors for keratinocytes in epidermal suprabasal keratinocytes and/or dermal fibroblasts .
	manualset3
190379	15	415570	7	NULL	NULL	0	NULL	keratinocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical treatment of skin with all-trans-retinoic acid ( ATRA ) , the major biologically active form of vitamin A , results in hyperproliferation of basal keratinocytes , leading to an accelerated turnover of epidermis cells and thickening of the epidermis , probably via induction of production of paracrine growth factors for keratinocytes in epidermal suprabasal keratinocytes and/or dermal fibroblasts .
	manualset3
190380	16	415570	7	NULL	NULL	0	NULL	epidermal suprabasal keratinocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical treatment of skin with all-trans-retinoic acid ( ATRA ) , the major biologically active form of vitamin A , results in hyperproliferation of basal keratinocytes , leading to an accelerated turnover of epidermis cells and thickening of the epidermis , probably via induction of production of paracrine growth factors for keratinocytes in epidermal suprabasal keratinocytes and/or dermal fibroblasts .
	manualset3
190381	17	415570	7	NULL	NULL	0	NULL	dermal fibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical treatment of skin with all-trans-retinoic acid ( ATRA ) , the major biologically active form of vitamin A , results in hyperproliferation of basal keratinocytes , leading to an accelerated turnover of epidermis cells and thickening of the epidermis , probably via induction of production of paracrine growth factors for keratinocytes in epidermal suprabasal keratinocytes and/or dermal fibroblasts .
	manualset3
190382	1	415571	7	NULL	NULL	0	NULL	Topical tretinoin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical tretinoin is of benefit in treating other forms of hyperpigmentation , for example liver spots , and we therefore investigated its effectiveness in melasma .
	manualset3
190383	2	415571	7	NULL	NULL	0	NULL	forms of hyperpigmentation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical tretinoin is of benefit in treating other forms of hyperpigmentation , for example liver spots , and we therefore investigated its effectiveness in melasma .
	manualset3
190384	3	415571	7	NULL	NULL	NULL	NULL	example	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Topical tretinoin is of benefit in treating other forms of hyperpigmentation , for example liver spots , and we therefore investigated its effectiveness in melasma .
	manualset3
190385	4	415571	7	NULL	NULL	0	NULL	liver spots	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical tretinoin is of benefit in treating other forms of hyperpigmentation , for example liver spots , and we therefore investigated its effectiveness in melasma .
	manualset3
190386	5	415571	7	NULL	NULL	0	NULL	effectiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical tretinoin is of benefit in treating other forms of hyperpigmentation , for example liver spots , and we therefore investigated its effectiveness in melasma .
	manualset3
190387	6	415571	7	NULL	NULL	0	NULL	melasma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Topical tretinoin is of benefit in treating other forms of hyperpigmentation , for example liver spots , and we therefore investigated its effectiveness in melasma .
	manualset3
190388	1	415572	7	NULL	NULL	0	NULL	Topics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Topics covered will be a brief overview of cytoskeletal mechanisms of migration , the role of ion channels and transporters involved in cell migration , and ways by which a polarized distribution of ion channels and transporters can be achieved in migrating cells .
	manualset3
190389	2	415572	7	NULL	NULL	0	NULL	overview 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Topics covered will be a brief overview of cytoskeletal mechanisms of migration , the role of ion channels and transporters involved in cell migration , and ways by which a polarized distribution of ion channels and transporters can be achieved in migrating cells .
	manualset3
190390	3	415572	7	NULL	NULL	0	NULL	cytoskeletal mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Topics covered will be a brief overview of cytoskeletal mechanisms of migration , the role of ion channels and transporters involved in cell migration , and ways by which a polarized distribution of ion channels and transporters can be achieved in migrating cells .
	manualset3
190391	4	415572	7	NULL	NULL	0	NULL	 migration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Topics covered will be a brief overview of cytoskeletal mechanisms of migration , the role of ion channels and transporters involved in cell migration , and ways by which a polarized distribution of ion channels and transporters can be achieved in migrating cells .
	manualset3
190392	5	415572	7	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Topics covered will be a brief overview of cytoskeletal mechanisms of migration , the role of ion channels and transporters involved in cell migration , and ways by which a polarized distribution of ion channels and transporters can be achieved in migrating cells .
	manualset3
190393	6	415572	7	NULL	NULL	0	NULL	 ion channels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Topics covered will be a brief overview of cytoskeletal mechanisms of migration , the role of ion channels and transporters involved in cell migration , and ways by which a polarized distribution of ion channels and transporters can be achieved in migrating cells .
	manualset3
190394	7	415572	7	NULL	NULL	0	NULL	 transporters	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Topics covered will be a brief overview of cytoskeletal mechanisms of migration , the role of ion channels and transporters involved in cell migration , and ways by which a polarized distribution of ion channels and transporters can be achieved in migrating cells .
	manualset3
190395	8	415572	7	NULL	NULL	0	NULL	cell migration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Topics covered will be a brief overview of cytoskeletal mechanisms of migration , the role of ion channels and transporters involved in cell migration , and ways by which a polarized distribution of ion channels and transporters can be achieved in migrating cells .
	manualset3
190396	9	415572	7	NULL	NULL	0	NULL	polarized distribution 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Topics covered will be a brief overview of cytoskeletal mechanisms of migration , the role of ion channels and transporters involved in cell migration , and ways by which a polarized distribution of ion channels and transporters can be achieved in migrating cells .
	manualset3
190397	10	415572	7	NULL	NULL	0	NULL	ion channels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Topics covered will be a brief overview of cytoskeletal mechanisms of migration , the role of ion channels and transporters involved in cell migration , and ways by which a polarized distribution of ion channels and transporters can be achieved in migrating cells .
	manualset3
190398	11	415572	7	NULL	NULL	0	NULL	transporters 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Topics covered will be a brief overview of cytoskeletal mechanisms of migration , the role of ion channels and transporters involved in cell migration , and ways by which a polarized distribution of ion channels and transporters can be achieved in migrating cells .
	manualset3
190399	12	415572	7	NULL	NULL	0	NULL	migrating cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Topics covered will be a brief overview of cytoskeletal mechanisms of migration , the role of ion channels and transporters involved in cell migration , and ways by which a polarized distribution of ion channels and transporters can be achieved in migrating cells .
	manualset3
190400	13	415572	7	NULL	NULL	0	NULL	ways	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Topics covered will be a brief overview of cytoskeletal mechanisms of migration , the role of ion channels and transporters involved in cell migration , and ways by which a polarized distribution of ion channels and transporters can be achieved in migrating cells .
	manualset3
190401	1	415573	7	NULL	NULL	0	NULL	Topiramate	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Topiramate in Lennox-Gastaut syndrome : open-label treatment of patients completing a randomized controlled trial .
	manualset3
190402	2	415573	7	NULL	NULL	0	NULL	Lennox-Gastaut syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Topiramate in Lennox-Gastaut syndrome : open-label treatment of patients completing a randomized controlled trial .
	manualset3
190403	3	415573	7	NULL	NULL	0	NULL	open-label treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Topiramate in Lennox-Gastaut syndrome : open-label treatment of patients completing a randomized controlled trial .
	manualset3
190404	4	415573	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Topiramate in Lennox-Gastaut syndrome : open-label treatment of patients completing a randomized controlled trial .
	manualset3
190405	5	415573	7	NULL	NULL	0	NULL	randomized controlled trial	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Topiramate in Lennox-Gastaut syndrome : open-label treatment of patients completing a randomized controlled trial .
	manualset3
190406	1	415574	7	NULL	NULL	0	NULL	Topographic mapping	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Topographic mapping of rapid transitions in EEG multiple frequencies : EEG frequency domain of operational synchrony .
	manualset3
190407	2	415574	7	NULL	NULL	0	NULL	rapid transitions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Topographic mapping of rapid transitions in EEG multiple frequencies : EEG frequency domain of operational synchrony .
	manualset3
190408	3	415574	7	NULL	NULL	0	NULL	EEG multiple frequencies	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Topographic mapping of rapid transitions in EEG multiple frequencies : EEG frequency domain of operational synchrony .
	manualset3
190409	4	415574	7	NULL	NULL	0	NULL	EEG frequency domain	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Topographic mapping of rapid transitions in EEG multiple frequencies : EEG frequency domain of operational synchrony .
	manualset3
190410	5	415574	7	NULL	NULL	0	NULL	operational synchrony	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Topographic mapping of rapid transitions in EEG multiple frequencies : EEG frequency domain of operational synchrony .
	manualset3
190411	1	415575	7	NULL	NULL	0	NULL	Topographical organization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Topographical organization of projections from the nucleus isthmi magnocellularis to the optic tectum of the chick brain .
	manualset3
190412	2	415575	7	NULL	NULL	0	NULL	projections	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Topographical organization of projections from the nucleus isthmi magnocellularis to the optic tectum of the chick brain .
	manualset3
190413	3	415575	7	NULL	NULL	0	NULL	 nucleus isthmi magnocellularis	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Topographical organization of projections from the nucleus isthmi magnocellularis to the optic tectum of the chick brain .
	manualset3
190414	4	415575	7	NULL	NULL	0	NULL	optic tectum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Topographical organization of projections from the nucleus isthmi magnocellularis to the optic tectum of the chick brain .
	manualset3
190415	5	415575	7	NULL	NULL	0	NULL	chick brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Topographical organization of projections from the nucleus isthmi magnocellularis to the optic tectum of the chick brain .
	manualset3
190416	1	415576	7	NULL	NULL	0	NULL	Topography	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Topography of spatially enhanced human short-latency somatosensory evoked potentials .
	manualset3
190417	2	415576	7	NULL	NULL	0	NULL	spatially enhanced human short-latency somatosensory evoked potentials	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Topography of spatially enhanced human short-latency somatosensory evoked potentials .
	manualset3
190420	1	415577	7	NULL	NULL	0	NULL	Topology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Topology of the plastid Ndh complex and its NDH-F subunit in thylakoid membranes .
	manualset3
190421	2	415577	7	NULL	NULL	NULL	NULL	plastid Ndh complex 	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Topology of the plastid Ndh complex and its NDH-F subunit in thylakoid membranes .
	manualset3
190581	3	415577	7	NULL	NULL	0	NULL	NDH-F subunit	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Topology of the plastid Ndh complex and its NDH-F subunit in thylakoid membranes .
	manualset3
190595	4	415577	7	NULL	NULL	0	NULL	thylakoid membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Topology of the plastid Ndh complex and its NDH-F subunit in thylakoid membranes .
	manualset3
190596	1	415578	7	NULL	NULL	0	NULL	framboesial hamsters	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	After framboesial hamsters were treated with penicillin the mitogenic activities of their lymph node and spleen cells were similar to or slightly raised above those of controls .
	manualset3
190597	2	415578	7	NULL	NULL	0	NULL	penicillin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	After framboesial hamsters were treated with penicillin the mitogenic activities of their lymph node and spleen cells were similar to or slightly raised above those of controls .
	manualset3
190598	3	415578	7	NULL	NULL	0	NULL	mitogenic activities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After framboesial hamsters were treated with penicillin the mitogenic activities of their lymph node and spleen cells were similar to or slightly raised above those of controls .
	manualset3
190599	4	415578	7	NULL	NULL	0	NULL	lymph node	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After framboesial hamsters were treated with penicillin the mitogenic activities of their lymph node and spleen cells were similar to or slightly raised above those of controls .
	manualset3
190600	5	415578	7	NULL	NULL	0	NULL	spleen cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	After framboesial hamsters were treated with penicillin the mitogenic activities of their lymph node and spleen cells were similar to or slightly raised above those of controls .
	manualset3
190601	6	415578	7	NULL	NULL	0	NULL	controls	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	After framboesial hamsters were treated with penicillin the mitogenic activities of their lymph node and spleen cells were similar to or slightly raised above those of controls .
	manualset3
190602	1	415579	7	NULL	NULL	0	NULL	Total 3HdT incorporation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Total 3HdT incorporation within both experimental lymph node compartments became less than controls by day 15 even though experimental nodes had a larger mass. 3HdT incorporation per milligram tissue weight decreased in all tissue compartments of experimental animals by day 13 -- 14 .
	manualset3
190603	2	415579	7	NULL	NULL	0	NULL	experimental lymph node compartments	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Total 3HdT incorporation within both experimental lymph node compartments became less than controls by day 15 even though experimental nodes had a larger mass. 3HdT incorporation per milligram tissue weight decreased in all tissue compartments of experimental animals by day 13 -- 14 .
	manualset3
190604	3	415579	7	NULL	NULL	0	NULL	 controls	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Total 3HdT incorporation within both experimental lymph node compartments became less than controls by day 15 even though experimental nodes had a larger mass. 3HdT incorporation per milligram tissue weight decreased in all tissue compartments of experimental animals by day 13 -- 14 .
	manualset3
190605	4	415579	7	NULL	NULL	0	NULL	 day 15	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Total 3HdT incorporation within both experimental lymph node compartments became less than controls by day 15 even though experimental nodes had a larger mass. 3HdT incorporation per milligram tissue weight decreased in all tissue compartments of experimental animals by day 13 -- 14 .
	manualset3
190606	5	415579	7	NULL	NULL	0	NULL	experimental nodes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Total 3HdT incorporation within both experimental lymph node compartments became less than controls by day 15 even though experimental nodes had a larger mass. 3HdT incorporation per milligram tissue weight decreased in all tissue compartments of experimental animals by day 13 -- 14 .
	manualset3
190607	6	415579	7	NULL	NULL	0	NULL	3HdT incorporation per milligram tissue weight 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Total 3HdT incorporation within both experimental lymph node compartments became less than controls by day 15 even though experimental nodes had a larger mass. 3HdT incorporation per milligram tissue weight decreased in all tissue compartments of experimental animals by day 13 -- 14 .
	manualset3
190608	7	415579	7	NULL	NULL	0	NULL	 tissue compartments	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Total 3HdT incorporation within both experimental lymph node compartments became less than controls by day 15 even though experimental nodes had a larger mass. 3HdT incorporation per milligram tissue weight decreased in all tissue compartments of experimental animals by day 13 -- 14 .
	manualset3
190609	8	415579	7	NULL	NULL	0	NULL	experimental animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Total 3HdT incorporation within both experimental lymph node compartments became less than controls by day 15 even though experimental nodes had a larger mass. 3HdT incorporation per milligram tissue weight decreased in all tissue compartments of experimental animals by day 13 -- 14 .
	manualset3
190610	9	415579	7	NULL	NULL	0	NULL	day 13 -- 14	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Total 3HdT incorporation within both experimental lymph node compartments became less than controls by day 15 even though experimental nodes had a larger mass. 3HdT incorporation per milligram tissue weight decreased in all tissue compartments of experimental animals by day 13 -- 14 .
	manualset3
190626	10	415579	7	NULL	NULL	0	NULL	 larger mass	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Total 3HdT incorporation within both experimental lymph node compartments became less than controls by day 15 even though experimental nodes had a larger mass. 3HdT incorporation per milligram tissue weight decreased in all tissue compartments of experimental animals by day 13 -- 14 .
	manualset3
190631	1	415580	7	NULL	NULL	0	NULL	Total and inflammatory lesion counts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Total and inflammatory lesion counts were performed by the same investigator during the eight weeks of study at biweekly intervals .
	manualset3
190632	2	415580	7	NULL	NULL	0	NULL	 investigator 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Total and inflammatory lesion counts were performed by the same investigator during the eight weeks of study at biweekly intervals .
	manualset3
190635	3	415580	7	NULL	NULL	0	NULL	eight weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Total and inflammatory lesion counts were performed by the same investigator during the eight weeks of study at biweekly intervals .
	manualset3
190638	4	415580	7	NULL	NULL	NULL	NULL	study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Total and inflammatory lesion counts were performed by the same investigator during the eight weeks of study at biweekly intervals .
	manualset3
190639	5	415580	7	NULL	NULL	0	NULL	biweekly intervals	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Total and inflammatory lesion counts were performed by the same investigator during the eight weeks of study at biweekly intervals .
	manualset3
190648	1	415581	7	NULL	NULL	0	NULL	Total antioxidant status	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Total antioxidant status had a significant negative correlation with blood pressure .
	manualset3
190650	2	415581	7	NULL	NULL	0	NULL	negative correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Total antioxidant status had a significant negative correlation with blood pressure .
	manualset3
190651	3	415581	7	NULL	NULL	0	NULL	blood pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Total antioxidant status had a significant negative correlation with blood pressure .
	manualset3
190838	1	415582	7	NULL	NULL	0	NULL	Total body radiation therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Total body radiation therapy for disseminated lymphosarcoma : results of a pilot study .
	manualset3
190839	2	415582	7	NULL	NULL	0	NULL	disseminated lymphosarcoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Total body radiation therapy for disseminated lymphosarcoma : results of a pilot study .
	manualset3
190840	3	415582	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Total body radiation therapy for disseminated lymphosarcoma : results of a pilot study .
	manualset3
190841	4	415582	7	NULL	NULL	0	NULL	pilot study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Total body radiation therapy for disseminated lymphosarcoma : results of a pilot study .
	manualset3
190842	1	415583	7	NULL	NULL	0	NULL	Total duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Total duration of coma and weekly Glasgow Coma Scale Scores were recorded for the two groups .
	manualset3
190843	2	415583	7	NULL	NULL	0	NULL	coma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Total duration of coma and weekly Glasgow Coma Scale Scores were recorded for the two groups .
	manualset3
190844	3	415583	7	NULL	NULL	0	NULL	weekly Glasgow Coma Scale Scores	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Total duration of coma and weekly Glasgow Coma Scale Scores were recorded for the two groups .
	manualset3
190845	4	415583	7	NULL	NULL	0	NULL	 two groups 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Total duration of coma and weekly Glasgow Coma Scale Scores were recorded for the two groups .
	manualset3
190846	1	415584	7	NULL	NULL	0	NULL	Total generation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Total generation and extracellular release of ROS by patients ' cells were significantly greater than those from controls after FcgammaR-stimulation , with ( P = 0.023 ) and without ( P & lt ; or = 0.023 ) priming with GM-CSF .
	manualset3
190847	2	415584	7	NULL	NULL	0	NULL	extracellular release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Total generation and extracellular release of ROS by patients ' cells were significantly greater than those from controls after FcgammaR-stimulation , with ( P = 0.023 ) and without ( P & lt ; or = 0.023 ) priming with GM-CSF .
	manualset3
190848	3	415584	7	NULL	NULL	0	NULL	ROS	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Total generation and extracellular release of ROS by patients ' cells were significantly greater than those from controls after FcgammaR-stimulation , with ( P = 0.023 ) and without ( P & lt ; or = 0.023 ) priming with GM-CSF .
	manualset3
190849	4	415584	7	NULL	NULL	0	NULL	patients ' cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Total generation and extracellular release of ROS by patients ' cells were significantly greater than those from controls after FcgammaR-stimulation , with ( P = 0.023 ) and without ( P & lt ; or = 0.023 ) priming with GM-CSF .
	manualset3
190850	5	415584	7	NULL	NULL	0	NULL	 controls	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Total generation and extracellular release of ROS by patients ' cells were significantly greater than those from controls after FcgammaR-stimulation , with ( P = 0.023 ) and without ( P & lt ; or = 0.023 ) priming with GM-CSF .
	manualset3
190851	6	415584	7	NULL	NULL	0	NULL	FcgammaR-stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Total generation and extracellular release of ROS by patients ' cells were significantly greater than those from controls after FcgammaR-stimulation , with ( P = 0.023 ) and without ( P & lt ; or = 0.023 ) priming with GM-CSF .
	manualset3
190852	7	415584	7	NULL	NULL	0	NULL	P = 0.023	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Total generation and extracellular release of ROS by patients ' cells were significantly greater than those from controls after FcgammaR-stimulation , with ( P = 0.023 ) and without ( P & lt ; or = 0.023 ) priming with GM-CSF .
	manualset3
190853	8	415584	7	NULL	NULL	0	NULL	P & lt ; or = 0.023	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Total generation and extracellular release of ROS by patients ' cells were significantly greater than those from controls after FcgammaR-stimulation , with ( P = 0.023 ) and without ( P & lt ; or = 0.023 ) priming with GM-CSF .
	manualset3
190854	9	415584	7	NULL	NULL	0	NULL	GM-CSF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Total generation and extracellular release of ROS by patients ' cells were significantly greater than those from controls after FcgammaR-stimulation , with ( P = 0.023 ) and without ( P & lt ; or = 0.023 ) priming with GM-CSF .
	manualset3
190855	1	415585	7	NULL	NULL	0	NULL	Total homocysteine ( tHCY )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Total homocysteine ( tHCY ) and folate are interrelated biomarkers for arteriosclerosis and coronary heart disease .
	manualset3
190856	2	415585	7	NULL	NULL	0	NULL	folate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Total homocysteine ( tHCY ) and folate are interrelated biomarkers for arteriosclerosis and coronary heart disease .
	manualset3
190857	3	415585	7	NULL	NULL	0	NULL	interrelated biomarkers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Total homocysteine ( tHCY ) and folate are interrelated biomarkers for arteriosclerosis and coronary heart disease .
	manualset3
190858	4	415585	7	NULL	NULL	0	NULL	arteriosclerosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Total homocysteine ( tHCY ) and folate are interrelated biomarkers for arteriosclerosis and coronary heart disease .
	manualset3
190859	5	415585	7	NULL	NULL	0	NULL	coronary heart disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Total homocysteine ( tHCY ) and folate are interrelated biomarkers for arteriosclerosis and coronary heart disease .
	manualset3
190860	1	415586	7	NULL	NULL	0	NULL	Total integration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Total integration of an ocular implant/prosthesis : preliminary in vivo study of a new design .
	manualset3
190861	2	415586	7	NULL	NULL	0	NULL	ocular implant/prosthesis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Total integration of an ocular implant/prosthesis : preliminary in vivo study of a new design .
	manualset3
190862	3	415586	7	NULL	NULL	0	NULL	in vivo study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Total integration of an ocular implant/prosthesis : preliminary in vivo study of a new design .
	manualset3
190863	4	415586	7	NULL	NULL	NULL	NULL	new design	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Total integration of an ocular implant/prosthesis : preliminary in vivo study of a new design .
	manualset3
190864	1	415587	7	NULL	NULL	0	NULL	Total internal reflection fluorescence microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Total internal reflection fluorescence microscopy revealed that mAbp1 formed propagating waves toward the front of the lamellipodium , which are characteristic for dynamic reorganization of the cytoskeleton .
	manualset3
190865	2	415587	7	NULL	NULL	0	NULL	mAbp1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Total internal reflection fluorescence microscopy revealed that mAbp1 formed propagating waves toward the front of the lamellipodium , which are characteristic for dynamic reorganization of the cytoskeleton .
	manualset3
190866	3	415587	7	NULL	NULL	0	NULL	propagating waves	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Total internal reflection fluorescence microscopy revealed that mAbp1 formed propagating waves toward the front of the lamellipodium , which are characteristic for dynamic reorganization of the cytoskeleton .
	manualset3
190867	4	415587	7	NULL	NULL	0	NULL	front of the lamellipodium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Total internal reflection fluorescence microscopy revealed that mAbp1 formed propagating waves toward the front of the lamellipodium , which are characteristic for dynamic reorganization of the cytoskeleton .
	manualset3
190868	5	415587	7	NULL	NULL	0	NULL	dynamic reorganization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Total internal reflection fluorescence microscopy revealed that mAbp1 formed propagating waves toward the front of the lamellipodium , which are characteristic for dynamic reorganization of the cytoskeleton .
	manualset3
190869	6	415587	7	NULL	NULL	0	NULL	cytoskeleton	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Total internal reflection fluorescence microscopy revealed that mAbp1 formed propagating waves toward the front of the lamellipodium , which are characteristic for dynamic reorganization of the cytoskeleton .
	manualset3
190870	1	415588	7	NULL	NULL	0	NULL	Total lymphocyte counts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Total lymphocyte and T cell counts were similar between the two groups .
	manualset3
190871	2	415588	7	NULL	NULL	0	NULL	 T cell counts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Total lymphocyte and T cell counts were similar between the two groups .
	manualset3
190872	3	415588	7	NULL	NULL	0	NULL	two groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Total lymphocyte and T cell counts were similar between the two groups .
	manualset3
190873	1	415589	7	NULL	NULL	NULL	NULL	Total n-3 fatty acids concentrations	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Total n-3 fatty acids ( p & lt ; 0.02 ) and hematin ( p & lt ; 0.0001 ) concentrations were significantly higher in muscle from pigs fed extensively than when fed in confinement .
	manualset3
190874	2	415589	7	NULL	NULL	0	NULL	p & lt ; 0.02	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Total n-3 fatty acids ( p & lt ; 0.02 ) and hematin ( p & lt ; 0.0001 ) concentrations were significantly higher in muscle from pigs fed extensively than when fed in confinement .
	manualset3
190875	3	415589	7	NULL	NULL	NULL	NULL	hematin concentrations	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Total n-3 fatty acids ( p & lt ; 0.02 ) and hematin ( p & lt ; 0.0001 ) concentrations were significantly higher in muscle from pigs fed extensively than when fed in confinement .
	manualset3
190876	4	415589	7	NULL	NULL	0	NULL	p & lt ; 0.0001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Total n-3 fatty acids ( p & lt ; 0.02 ) and hematin ( p & lt ; 0.0001 ) concentrations were significantly higher in muscle from pigs fed extensively than when fed in confinement .
	manualset3
190877	5	415589	7	NULL	NULL	0	NULL	muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Total n-3 fatty acids ( p & lt ; 0.02 ) and hematin ( p & lt ; 0.0001 ) concentrations were significantly higher in muscle from pigs fed extensively than when fed in confinement .
	manualset3
190878	6	415589	7	NULL	NULL	0	NULL	pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Total n-3 fatty acids ( p & lt ; 0.02 ) and hematin ( p & lt ; 0.0001 ) concentrations were significantly higher in muscle from pigs fed extensively than when fed in confinement .
	manualset3
190879	7	415589	7	NULL	NULL	0	NULL	confinement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Total n-3 fatty acids ( p & lt ; 0.02 ) and hematin ( p & lt ; 0.0001 ) concentrations were significantly higher in muscle from pigs fed extensively than when fed in confinement .
	manualset3
190880	1	415590	7	NULL	NULL	0	NULL	Total organic halogen ( TOX )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Total organic halogen ( TOX ) is a collective parameter and a toxicity indicator for all the halogenated organic disinfection byproducts ( DBPs ) in a water sample .
	manualset3
190881	2	415590	7	NULL	NULL	0	NULL	collective parameter	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Total organic halogen ( TOX ) is a collective parameter and a toxicity indicator for all the halogenated organic disinfection byproducts ( DBPs ) in a water sample .
	manualset3
190882	3	415590	7	NULL	NULL	0	NULL	toxicity indicator	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Total organic halogen ( TOX ) is a collective parameter and a toxicity indicator for all the halogenated organic disinfection byproducts ( DBPs ) in a water sample .
	manualset3
190883	4	415590	7	NULL	NULL	0	NULL	halogenated organic disinfection byproducts ( DBPs )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Total organic halogen ( TOX ) is a collective parameter and a toxicity indicator for all the halogenated organic disinfection byproducts ( DBPs ) in a water sample .
	manualset3
190884	5	415590	7	NULL	NULL	0	NULL	 water sample	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Total organic halogen ( TOX ) is a collective parameter and a toxicity indicator for all the halogenated organic disinfection byproducts ( DBPs ) in a water sample .
	manualset3
190885	1	415591	7	NULL	NULL	0	NULL	Total pancreatic RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Total pancreatic RNA from the holocephalan species Callorhyncus milii ( elephantfish ) was used to make cDNA as a template for the polymerase chain reaction .
	manualset3
190886	2	415591	7	NULL	NULL	0	NULL	holocephalan species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Total pancreatic RNA from the holocephalan species Callorhyncus milii ( elephantfish ) was used to make cDNA as a template for the polymerase chain reaction .
	manualset3
190887	3	415591	7	NULL	NULL	0	NULL	Callorhyncus milii ( elephantfish ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Total pancreatic RNA from the holocephalan species Callorhyncus milii ( elephantfish ) was used to make cDNA as a template for the polymerase chain reaction .
	manualset3
190888	4	415591	7	NULL	NULL	0	NULL	cDNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Total pancreatic RNA from the holocephalan species Callorhyncus milii ( elephantfish ) was used to make cDNA as a template for the polymerase chain reaction .
	manualset3
190889	5	415591	7	NULL	NULL	0	NULL	template 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Total pancreatic RNA from the holocephalan species Callorhyncus milii ( elephantfish ) was used to make cDNA as a template for the polymerase chain reaction .
	manualset3
190890	6	415591	7	NULL	NULL	0	NULL	polymerase chain reaction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Total pancreatic RNA from the holocephalan species Callorhyncus milii ( elephantfish ) was used to make cDNA as a template for the polymerase chain reaction .
	manualset3
190892	1	415592	7	NULL	NULL	0	NULL	Total parenteral nutrition-associated cholestasis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Total parenteral nutrition-associated cholestasis : acute studies in infant and adult rabbits .
	manualset3
190893	2	415592	7	NULL	NULL	0	NULL	acute studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Total parenteral nutrition-associated cholestasis : acute studies in infant and adult rabbits .
	manualset3
190899	3	415592	7	NULL	NULL	0	NULL	 infant rabbits	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Total parenteral nutrition-associated cholestasis : acute studies in infant and adult rabbits .
	manualset3
190901	4	415592	7	NULL	NULL	0	NULL	adult rabbits	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Total parenteral nutrition-associated cholestasis : acute studies in infant and adult rabbits .
	manualset3
190908	1	415593	7	NULL	NULL	0	NULL	Total pituitary RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Total pituitary RNA was extracted on embryonic days ( e - ) 11 , 13 , 15 , 17 , and 19 and neonatal days ( d - ) 1 , 3 , 6 , 9 , and 12 and subjected to ribonuclease protection assays ( RPA ) for chicken TSHbeta mRNA .
	manualset3
190909	2	415593	7	NULL	NULL	0	NULL	embryonic days ( e - )	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Total pituitary RNA was extracted on embryonic days ( e - ) 11 , 13 , 15 , 17 , and 19 and neonatal days ( d - ) 1 , 3 , 6 , 9 , and 12 and subjected to ribonuclease protection assays ( RPA ) for chicken TSHbeta mRNA .
	manualset3
190910	3	415593	7	NULL	NULL	NULL	NULL	11	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Total pituitary RNA was extracted on embryonic days ( e - ) 11 , 13 , 15 , 17 , and 19 and neonatal days ( d - ) 1 , 3 , 6 , 9 , and 12 and subjected to ribonuclease protection assays ( RPA ) for chicken TSHbeta mRNA .
	manualset3
190911	4	415593	7	NULL	NULL	NULL	NULL	13	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Total pituitary RNA was extracted on embryonic days ( e - ) 11 , 13 , 15 , 17 , and 19 and neonatal days ( d - ) 1 , 3 , 6 , 9 , and 12 and subjected to ribonuclease protection assays ( RPA ) for chicken TSHbeta mRNA .
	manualset3
190913	5	415593	7	NULL	NULL	NULL	NULL	15	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Total pituitary RNA was extracted on embryonic days ( e - ) 11 , 13 , 15 , 17 , and 19 and neonatal days ( d - ) 1 , 3 , 6 , 9 , and 12 and subjected to ribonuclease protection assays ( RPA ) for chicken TSHbeta mRNA .
	manualset3
190915	6	415593	7	NULL	NULL	NULL	NULL	17	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Total pituitary RNA was extracted on embryonic days ( e - ) 11 , 13 , 15 , 17 , and 19 and neonatal days ( d - ) 1 , 3 , 6 , 9 , and 12 and subjected to ribonuclease protection assays ( RPA ) for chicken TSHbeta mRNA .
	manualset3
190919	7	415593	7	NULL	NULL	NULL	NULL	19	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Total pituitary RNA was extracted on embryonic days ( e - ) 11 , 13 , 15 , 17 , and 19 and neonatal days ( d - ) 1 , 3 , 6 , 9 , and 12 and subjected to ribonuclease protection assays ( RPA ) for chicken TSHbeta mRNA .
	manualset3
190922	8	415593	7	NULL	NULL	NULL	NULL	 neonatal days ( d - )	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Total pituitary RNA was extracted on embryonic days ( e - ) 11 , 13 , 15 , 17 , and 19 and neonatal days ( d - ) 1 , 3 , 6 , 9 , and 12 and subjected to ribonuclease protection assays ( RPA ) for chicken TSHbeta mRNA .
	manualset3
190923	9	415593	7	NULL	NULL	NULL	NULL	1 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Total pituitary RNA was extracted on embryonic days ( e - ) 11 , 13 , 15 , 17 , and 19 and neonatal days ( d - ) 1 , 3 , 6 , 9 , and 12 and subjected to ribonuclease protection assays ( RPA ) for chicken TSHbeta mRNA .
	manualset3
190927	10	415593	7	NULL	NULL	0	NULL	3 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Total pituitary RNA was extracted on embryonic days ( e - ) 11 , 13 , 15 , 17 , and 19 and neonatal days ( d - ) 1 , 3 , 6 , 9 , and 12 and subjected to ribonuclease protection assays ( RPA ) for chicken TSHbeta mRNA .
	manualset3
190932	11	415593	7	NULL	NULL	0	NULL	6	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Total pituitary RNA was extracted on embryonic days ( e - ) 11 , 13 , 15 , 17 , and 19 and neonatal days ( d - ) 1 , 3 , 6 , 9 , and 12 and subjected to ribonuclease protection assays ( RPA ) for chicken TSHbeta mRNA .
	manualset3
190934	12	415593	7	NULL	NULL	0	NULL	9	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Total pituitary RNA was extracted on embryonic days ( e - ) 11 , 13 , 15 , 17 , and 19 and neonatal days ( d - ) 1 , 3 , 6 , 9 , and 12 and subjected to ribonuclease protection assays ( RPA ) for chicken TSHbeta mRNA .
	manualset3
190937	13	415593	7	NULL	NULL	0	NULL	12 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Total pituitary RNA was extracted on embryonic days ( e - ) 11 , 13 , 15 , 17 , and 19 and neonatal days ( d - ) 1 , 3 , 6 , 9 , and 12 and subjected to ribonuclease protection assays ( RPA ) for chicken TSHbeta mRNA .
	manualset3
190940	14	415593	7	NULL	NULL	0	NULL	ribonuclease protection assays ( RPA )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Total pituitary RNA was extracted on embryonic days ( e - ) 11 , 13 , 15 , 17 , and 19 and neonatal days ( d - ) 1 , 3 , 6 , 9 , and 12 and subjected to ribonuclease protection assays ( RPA ) for chicken TSHbeta mRNA .
	manualset3
190942	15	415593	7	NULL	NULL	0	NULL	chicken TSHbeta mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Total pituitary RNA was extracted on embryonic days ( e - ) 11 , 13 , 15 , 17 , and 19 and neonatal days ( d - ) 1 , 3 , 6 , 9 , and 12 and subjected to ribonuclease protection assays ( RPA ) for chicken TSHbeta mRNA .
	manualset3
190948	1	415594	7	NULL	NULL	0	NULL	Total prevalence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Total prevalence was 1.47 per 100 , 000 births ( 95 % CI : 1.32-1 .62 ) .
	manualset3
190949	2	415594	7	NULL	NULL	0	NULL	1.47 per 100 , 000 births	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Total prevalence was 1.47 per 100 , 000 births ( 95 % CI : 1.32-1 .62 ) .
	manualset3
190951	3	415594	7	NULL	NULL	0	NULL	95 % CI : 1.32-1 .62	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Total prevalence was 1.47 per 100 , 000 births ( 95 % CI : 1.32-1 .62 ) .
	manualset3
190968	1	415595	7	NULL	NULL	0	NULL	Total protein extracts	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Total protein extracts immunoprecipitated with a CDC27a antibody showed ubiquitin ligase activity , indicating that the Arabidopsis CDC27a gets incorporated into APC complexes .
	manualset3
190969	2	415595	7	NULL	NULL	0	NULL	CDC27a antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Total protein extracts immunoprecipitated with a CDC27a antibody showed ubiquitin ligase activity , indicating that the Arabidopsis CDC27a gets incorporated into APC complexes .
	manualset3
190970	3	415595	7	NULL	NULL	0	NULL	ubiquitin ligase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Total protein extracts immunoprecipitated with a CDC27a antibody showed ubiquitin ligase activity , indicating that the Arabidopsis CDC27a gets incorporated into APC complexes .
	manualset3
190971	4	415595	7	NULL	NULL	0	NULL	Arabidopsis CDC27a	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Total protein extracts immunoprecipitated with a CDC27a antibody showed ubiquitin ligase activity , indicating that the Arabidopsis CDC27a gets incorporated into APC complexes .
	manualset3
190972	5	415595	7	NULL	NULL	0	NULL	APC complexes	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Total protein extracts immunoprecipitated with a CDC27a antibody showed ubiquitin ligase activity , indicating that the Arabidopsis CDC27a gets incorporated into APC complexes .
	manualset3
190973	1	415596	7	NULL	NULL	0	NULL	Total sleep deprivation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Total sleep deprivation has been widely researched , and its effects have been well described .
	manualset3
190974	2	415596	7	NULL	NULL	0	NULL	effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Total sleep deprivation has been widely researched , and its effects have been well described .
	manualset3
190986	1	415597	7	NULL	NULL	0	NULL	Total tract apparent digestibilities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Total tract apparent digestibilities of DM , CP , and starch were greater for su-Bn2 diets .
	manualset3
190987	2	415597	7	NULL	NULL	0	NULL	DM	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Total tract apparent digestibilities of DM , CP , and starch were greater for su-Bn2 diets .
	manualset3
190988	3	415597	7	NULL	NULL	0	NULL	CP	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Total tract apparent digestibilities of DM , CP , and starch were greater for su-Bn2 diets .
	manualset3
190989	4	415597	7	NULL	NULL	0	NULL	starch	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Total tract apparent digestibilities of DM , CP , and starch were greater for su-Bn2 diets .
	manualset3
190990	5	415597	7	NULL	NULL	0	NULL	su-Bn2 diets	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Total tract apparent digestibilities of DM , CP , and starch were greater for su-Bn2 diets .
	manualset3
190994	1	415598	7	NULL	NULL	0	NULL	efficient synthesis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Toward an efficient synthesis of taxane analogs by dienyne ring-closing metathesis .
	manualset3
190996	2	415598	7	NULL	NULL	0	NULL	taxane analogs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Toward an efficient synthesis of taxane analogs by dienyne ring-closing metathesis .
	manualset3
190999	3	415598	7	NULL	NULL	0	NULL	dienyne ring-closing metathesis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Toward an efficient synthesis of taxane analogs by dienyne ring-closing metathesis .
	manualset3
191000	1	415599	7	NULL	NULL	0	NULL	parturition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Towards parturition , no changes in PR mRNA levels were recorded in the UUS , whereas the LUS displayed a gradual increase .
	manualset3
191001	2	415599	7	NULL	NULL	0	NULL	changes 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Towards parturition , no changes in PR mRNA levels were recorded in the UUS , whereas the LUS displayed a gradual increase .
	manualset3
191002	3	415599	7	NULL	NULL	0	NULL	PR mRNA levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Towards parturition , no changes in PR mRNA levels were recorded in the UUS , whereas the LUS displayed a gradual increase .
	manualset3
191003	4	415599	7	NULL	NULL	0	NULL	UUS	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Towards parturition , no changes in PR mRNA levels were recorded in the UUS , whereas the LUS displayed a gradual increase .
	manualset3
191006	5	415599	7	NULL	NULL	0	NULL	LUS	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Towards parturition , no changes in PR mRNA levels were recorded in the UUS , whereas the LUS displayed a gradual increase .
	manualset3
191008	6	415599	7	NULL	NULL	0	NULL	gradual increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Towards parturition , no changes in PR mRNA levels were recorded in the UUS , whereas the LUS displayed a gradual increase .
	manualset3
191028	1	415600	7	NULL	NULL	0	NULL	Toxemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxemia at the same time promotes the increase of hematoencephalic barrier permeability , intake of inflammatory cytokines into the brain that induce inflammation in the brain periventricular areas with the development of intestinal encephalopathy .
	manualset3
191030	2	415600	7	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxemia at the same time promotes the increase of hematoencephalic barrier permeability , intake of inflammatory cytokines into the brain that induce inflammation in the brain periventricular areas with the development of intestinal encephalopathy .
	manualset3
191033	3	415600	7	NULL	NULL	0	NULL	increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxemia at the same time promotes the increase of hematoencephalic barrier permeability , intake of inflammatory cytokines into the brain that induce inflammation in the brain periventricular areas with the development of intestinal encephalopathy .
	manualset3
191035	4	415600	7	NULL	NULL	0	NULL	hematoencephalic barrier permeability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxemia at the same time promotes the increase of hematoencephalic barrier permeability , intake of inflammatory cytokines into the brain that induce inflammation in the brain periventricular areas with the development of intestinal encephalopathy .
	manualset3
191040	5	415600	7	NULL	NULL	0	NULL	intake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxemia at the same time promotes the increase of hematoencephalic barrier permeability , intake of inflammatory cytokines into the brain that induce inflammation in the brain periventricular areas with the development of intestinal encephalopathy .
	manualset3
191042	6	415600	7	NULL	NULL	0	NULL	inflammatory cytokines	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxemia at the same time promotes the increase of hematoencephalic barrier permeability , intake of inflammatory cytokines into the brain that induce inflammation in the brain periventricular areas with the development of intestinal encephalopathy .
	manualset3
191043	7	415600	7	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxemia at the same time promotes the increase of hematoencephalic barrier permeability , intake of inflammatory cytokines into the brain that induce inflammation in the brain periventricular areas with the development of intestinal encephalopathy .
	manualset3
191044	8	415600	7	NULL	NULL	0	NULL	inflammation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxemia at the same time promotes the increase of hematoencephalic barrier permeability , intake of inflammatory cytokines into the brain that induce inflammation in the brain periventricular areas with the development of intestinal encephalopathy .
	manualset3
191047	9	415600	7	NULL	NULL	0	NULL	brain periventricular areas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxemia at the same time promotes the increase of hematoencephalic barrier permeability , intake of inflammatory cytokines into the brain that induce inflammation in the brain periventricular areas with the development of intestinal encephalopathy .
	manualset3
191050	10	415600	7	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxemia at the same time promotes the increase of hematoencephalic barrier permeability , intake of inflammatory cytokines into the brain that induce inflammation in the brain periventricular areas with the development of intestinal encephalopathy .
	manualset3
191051	11	415600	7	NULL	NULL	0	NULL	 intestinal encephalopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxemia at the same time promotes the increase of hematoencephalic barrier permeability , intake of inflammatory cytokines into the brain that induce inflammation in the brain periventricular areas with the development of intestinal encephalopathy .
	manualset3
191058	1	415601	7	NULL	NULL	NULL	NULL	Toxic epidermal necrolysis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Toxic epidermal necrolysis secondary to carbamazepine in a patient with human immunodeficiency virus infection .
	manualset3
191059	2	415601	7	NULL	NULL	0	NULL	carbamazepine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxic epidermal necrolysis secondary to carbamazepine in a patient with human immunodeficiency virus infection .
	manualset3
191075	3	415601	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxic epidermal necrolysis secondary to carbamazepine in a patient with human immunodeficiency virus infection .
	manualset3
191076	4	415601	7	NULL	NULL	NULL	NULL	human immunodeficiency virus infection	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Toxic epidermal necrolysis secondary to carbamazepine in a patient with human immunodeficiency virus infection .
	manualset3
191095	1	415602	7	NULL	NULL	0	NULL	Toxic hygroscopic contact reaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxic hygroscopic contact reaction to N-methyl-2-pyrrolidone .
	manualset3
191096	2	415602	7	NULL	NULL	0	NULL	N-methyl-2-pyrrolidone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxic hygroscopic contact reaction to N-methyl-2-pyrrolidone .
	manualset3
191131	1	415603	7	NULL	NULL	0	NULL	histopathological evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After histopathological evaluation , deparafinisation and lysis of the specimens , one-stage polymerase chain reaction ( PCR ) and two-stage ( nested ) PCR assays were performed with the primers common for both EBV genotypes and the primers specific for EBV types 1 and 2 , respectively .
	manualset3
191132	2	415603	7	NULL	NULL	0	NULL	 deparafinisation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After histopathological evaluation , deparafinisation and lysis of the specimens , one-stage polymerase chain reaction ( PCR ) and two-stage ( nested ) PCR assays were performed with the primers common for both EBV genotypes and the primers specific for EBV types 1 and 2 , respectively .
	manualset3
191133	3	415603	7	NULL	NULL	0	NULL	 lysis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After histopathological evaluation , deparafinisation and lysis of the specimens , one-stage polymerase chain reaction ( PCR ) and two-stage ( nested ) PCR assays were performed with the primers common for both EBV genotypes and the primers specific for EBV types 1 and 2 , respectively .
	manualset3
191134	4	415603	7	NULL	NULL	0	NULL	specimens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	After histopathological evaluation , deparafinisation and lysis of the specimens , one-stage polymerase chain reaction ( PCR ) and two-stage ( nested ) PCR assays were performed with the primers common for both EBV genotypes and the primers specific for EBV types 1 and 2 , respectively .
	manualset3
191135	5	415603	7	NULL	NULL	0	NULL	one-stage polymerase chain reaction ( PCR )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After histopathological evaluation , deparafinisation and lysis of the specimens , one-stage polymerase chain reaction ( PCR ) and two-stage ( nested ) PCR assays were performed with the primers common for both EBV genotypes and the primers specific for EBV types 1 and 2 , respectively .
	manualset3
191136	6	415603	7	NULL	NULL	0	NULL	two-stage ( nested ) PCR assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After histopathological evaluation , deparafinisation and lysis of the specimens , one-stage polymerase chain reaction ( PCR ) and two-stage ( nested ) PCR assays were performed with the primers common for both EBV genotypes and the primers specific for EBV types 1 and 2 , respectively .
	manualset3
191137	7	415603	7	NULL	NULL	0	NULL	primers	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	After histopathological evaluation , deparafinisation and lysis of the specimens , one-stage polymerase chain reaction ( PCR ) and two-stage ( nested ) PCR assays were performed with the primers common for both EBV genotypes and the primers specific for EBV types 1 and 2 , respectively .
	manualset3
191138	8	415603	7	NULL	NULL	0	NULL	EBV genotypes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	After histopathological evaluation , deparafinisation and lysis of the specimens , one-stage polymerase chain reaction ( PCR ) and two-stage ( nested ) PCR assays were performed with the primers common for both EBV genotypes and the primers specific for EBV types 1 and 2 , respectively .
	manualset3
191139	9	415603	7	NULL	NULL	0	NULL	 primers	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	After histopathological evaluation , deparafinisation and lysis of the specimens , one-stage polymerase chain reaction ( PCR ) and two-stage ( nested ) PCR assays were performed with the primers common for both EBV genotypes and the primers specific for EBV types 1 and 2 , respectively .
	manualset3
191140	10	415603	7	NULL	NULL	0	NULL	EBV types 1	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	After histopathological evaluation , deparafinisation and lysis of the specimens , one-stage polymerase chain reaction ( PCR ) and two-stage ( nested ) PCR assays were performed with the primers common for both EBV genotypes and the primers specific for EBV types 1 and 2 , respectively .
	manualset3
191141	11	415603	7	NULL	NULL	0	NULL	EBV types 2	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	After histopathological evaluation , deparafinisation and lysis of the specimens , one-stage polymerase chain reaction ( PCR ) and two-stage ( nested ) PCR assays were performed with the primers common for both EBV genotypes and the primers specific for EBV types 1 and 2 , respectively .
	manualset3
191145	1	415604	7	NULL	NULL	0	NULL	Toxicant-induced epithelial lesions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicant-induced epithelial lesions in the nasal passages of laboratory animals ( and humans ) are often site-specific and dependent on the intranasal regional dose of the inhaled chemical and the sensitivity of the nasal epithelial tissue to the specific chemical .
	manualset3
191146	2	415604	7	NULL	NULL	0	NULL	nasal passages	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicant-induced epithelial lesions in the nasal passages of laboratory animals ( and humans ) are often site-specific and dependent on the intranasal regional dose of the inhaled chemical and the sensitivity of the nasal epithelial tissue to the specific chemical .
	manualset3
191147	3	415604	7	NULL	NULL	0	NULL	laboratory animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicant-induced epithelial lesions in the nasal passages of laboratory animals ( and humans ) are often site-specific and dependent on the intranasal regional dose of the inhaled chemical and the sensitivity of the nasal epithelial tissue to the specific chemical .
	manualset3
191148	4	415604	7	NULL	NULL	0	NULL	humans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicant-induced epithelial lesions in the nasal passages of laboratory animals ( and humans ) are often site-specific and dependent on the intranasal regional dose of the inhaled chemical and the sensitivity of the nasal epithelial tissue to the specific chemical .
	manualset3
191149	5	415604	7	NULL	NULL	0	NULL	 intranasal regional dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicant-induced epithelial lesions in the nasal passages of laboratory animals ( and humans ) are often site-specific and dependent on the intranasal regional dose of the inhaled chemical and the sensitivity of the nasal epithelial tissue to the specific chemical .
	manualset3
191150	6	415604	7	NULL	NULL	0	NULL	inhaled chemical	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicant-induced epithelial lesions in the nasal passages of laboratory animals ( and humans ) are often site-specific and dependent on the intranasal regional dose of the inhaled chemical and the sensitivity of the nasal epithelial tissue to the specific chemical .
	manualset3
191151	7	415604	7	NULL	NULL	0	NULL	sensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicant-induced epithelial lesions in the nasal passages of laboratory animals ( and humans ) are often site-specific and dependent on the intranasal regional dose of the inhaled chemical and the sensitivity of the nasal epithelial tissue to the specific chemical .
	manualset3
191152	8	415604	7	NULL	NULL	0	NULL	nasal epithelial tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicant-induced epithelial lesions in the nasal passages of laboratory animals ( and humans ) are often site-specific and dependent on the intranasal regional dose of the inhaled chemical and the sensitivity of the nasal epithelial tissue to the specific chemical .
	manualset3
191153	9	415604	7	NULL	NULL	0	NULL	chemical	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicant-induced epithelial lesions in the nasal passages of laboratory animals ( and humans ) are often site-specific and dependent on the intranasal regional dose of the inhaled chemical and the sensitivity of the nasal epithelial tissue to the specific chemical .
	manualset3
191154	1	415605	7	NULL	NULL	0	NULL	Toxicity assessment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicity assessment of zebrafish following exposure to CdTe QDs .
	manualset3
191155	2	415605	7	NULL	NULL	0	NULL	zebrafish	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicity assessment of zebrafish following exposure to CdTe QDs .
	manualset3
191156	3	415605	7	NULL	NULL	0	NULL	CdTe QDs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicity assessment of zebrafish following exposure to CdTe QDs .
	manualset3
193189	4	415605	7	NULL	NULL	0	NULL	exposure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicity assessment of zebrafish following exposure to CdTe QDs .
	manualset3
191157	1	415606	7	NULL	NULL	0	NULL	Toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicity in the CTX arm was tolerable .
	manualset3
191158	2	415606	7	NULL	NULL	0	NULL	CTX arm	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicity in the CTX arm was tolerable .
	manualset3
191159	1	415607	7	NULL	NULL	0	NULL	Toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicity of cadmium , cobalt , copper , zinc , nickel , lead , chromium , and arsenic at five different concentrations ( 0.01-1 mM ) was tested by standard ecotoxicity test .
	manualset3
191160	2	415607	7	NULL	NULL	0	NULL	cadmium 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicity of cadmium , cobalt , copper , zinc , nickel , lead , chromium , and arsenic at five different concentrations ( 0.01-1 mM ) was tested by standard ecotoxicity test .
	manualset3
191161	3	415607	7	NULL	NULL	0	NULL	cobalt 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicity of cadmium , cobalt , copper , zinc , nickel , lead , chromium , and arsenic at five different concentrations ( 0.01-1 mM ) was tested by standard ecotoxicity test .
	manualset3
191162	4	415607	7	NULL	NULL	0	NULL	copper	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicity of cadmium , cobalt , copper , zinc , nickel , lead , chromium , and arsenic at five different concentrations ( 0.01-1 mM ) was tested by standard ecotoxicity test .
	manualset3
191163	5	415607	7	NULL	NULL	0	NULL	zinc	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicity of cadmium , cobalt , copper , zinc , nickel , lead , chromium , and arsenic at five different concentrations ( 0.01-1 mM ) was tested by standard ecotoxicity test .
	manualset3
191164	6	415607	7	NULL	NULL	0	NULL	nickel	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicity of cadmium , cobalt , copper , zinc , nickel , lead , chromium , and arsenic at five different concentrations ( 0.01-1 mM ) was tested by standard ecotoxicity test .
	manualset3
191165	7	415607	7	NULL	NULL	0	NULL	lead	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicity of cadmium , cobalt , copper , zinc , nickel , lead , chromium , and arsenic at five different concentrations ( 0.01-1 mM ) was tested by standard ecotoxicity test .
	manualset3
191166	8	415607	7	NULL	NULL	0	NULL	chromium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicity of cadmium , cobalt , copper , zinc , nickel , lead , chromium , and arsenic at five different concentrations ( 0.01-1 mM ) was tested by standard ecotoxicity test .
	manualset3
191167	9	415607	7	NULL	NULL	0	NULL	arsenic	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicity of cadmium , cobalt , copper , zinc , nickel , lead , chromium , and arsenic at five different concentrations ( 0.01-1 mM ) was tested by standard ecotoxicity test .
	manualset3
191168	10	415607	7	NULL	NULL	0	NULL	five different concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicity of cadmium , cobalt , copper , zinc , nickel , lead , chromium , and arsenic at five different concentrations ( 0.01-1 mM ) was tested by standard ecotoxicity test .
	manualset3
191169	11	415607	7	NULL	NULL	0	NULL	0.01-1 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicity of cadmium , cobalt , copper , zinc , nickel , lead , chromium , and arsenic at five different concentrations ( 0.01-1 mM ) was tested by standard ecotoxicity test .
	manualset3
191170	12	415607	7	NULL	NULL	0	NULL	standard ecotoxicity test 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicity of cadmium , cobalt , copper , zinc , nickel , lead , chromium , and arsenic at five different concentrations ( 0.01-1 mM ) was tested by standard ecotoxicity test .
	manualset3
191171	1	415608	7	NULL	NULL	0	NULL	Toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicity was acceptable except for carboplatin with constant grade 4 leukocytes or platelets toxicity .
	manualset3
191172	2	415608	7	NULL	NULL	0	NULL	carboplatin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicity was acceptable except for carboplatin with constant grade 4 leukocytes or platelets toxicity .
	manualset3
191173	3	415608	7	NULL	NULL	0	NULL	constant grade 4 leukocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicity was acceptable except for carboplatin with constant grade 4 leukocytes or platelets toxicity .
	manualset3
191174	4	415608	7	NULL	NULL	0	NULL	platelets toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicity was acceptable except for carboplatin with constant grade 4 leukocytes or platelets toxicity .
	manualset3
191175	1	415609	7	NULL	NULL	0	NULL	Toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicity was assessed according to WHO criteria .
	manualset3
191176	2	415609	7	NULL	NULL	0	NULL	WHO criteria	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicity was assessed according to WHO criteria .
	manualset3
191177	1	415610	7	NULL	NULL	0	NULL	Toxin Bc2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxin Bc2 and EqTx-II were cytotoxic against human U87 and A172 GBM cell lines either wild type or p53 mutant , a tumor suppressor frequently mutated in malignant gliomas .
	manualset3
191178	2	415610	7	NULL	NULL	0	NULL	EqTx-II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxin Bc2 and EqTx-II were cytotoxic against human U87 and A172 GBM cell lines either wild type or p53 mutant , a tumor suppressor frequently mutated in malignant gliomas .
	manualset3
191179	3	415610	7	NULL	NULL	0	NULL	human U87 cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxin Bc2 and EqTx-II were cytotoxic against human U87 and A172 GBM cell lines either wild type or p53 mutant , a tumor suppressor frequently mutated in malignant gliomas .
	manualset3
191180	4	415610	7	NULL	NULL	0	NULL	A172 GBM cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxin Bc2 and EqTx-II were cytotoxic against human U87 and A172 GBM cell lines either wild type or p53 mutant , a tumor suppressor frequently mutated in malignant gliomas .
	manualset3
191181	5	415610	7	NULL	NULL	0	NULL	wild type	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxin Bc2 and EqTx-II were cytotoxic against human U87 and A172 GBM cell lines either wild type or p53 mutant , a tumor suppressor frequently mutated in malignant gliomas .
	manualset3
191182	6	415610	7	NULL	NULL	0	NULL	p53 mutant	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxin Bc2 and EqTx-II were cytotoxic against human U87 and A172 GBM cell lines either wild type or p53 mutant , a tumor suppressor frequently mutated in malignant gliomas .
	manualset3
191183	7	415610	7	NULL	NULL	0	NULL	 tumor suppressor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxin Bc2 and EqTx-II were cytotoxic against human U87 and A172 GBM cell lines either wild type or p53 mutant , a tumor suppressor frequently mutated in malignant gliomas .
	manualset3
191184	8	415610	7	NULL	NULL	0	NULL	malignant gliomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxin Bc2 and EqTx-II were cytotoxic against human U87 and A172 GBM cell lines either wild type or p53 mutant , a tumor suppressor frequently mutated in malignant gliomas .
	manualset3
191487	1	415611	7	NULL	NULL	0	NULL	Tracheal resection 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Tracheal resection was performed in 10 patients with non-malignant tracheal tumors .
	manualset3
191488	2	415611	7	NULL	NULL	0	NULL	10 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Tracheal resection was performed in 10 patients with non-malignant tracheal tumors .
	manualset3
191489	3	415611	7	NULL	NULL	0	NULL	non-malignant tracheal tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Tracheal resection was performed in 10 patients with non-malignant tracheal tumors .
	manualset3
191490	1	415612	7	NULL	NULL	0	NULL	Tracheobronchial clearance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Tracheobronchial clearance in health and disease : with special reference to interciliary fluid .
	manualset3
191491	2	415612	7	NULL	NULL	0	NULL	health 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Tracheobronchial clearance in health and disease : with special reference to interciliary fluid .
	manualset3
191492	3	415612	7	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Tracheobronchial clearance in health and disease : with special reference to interciliary fluid .
	manualset3
191493	4	415612	7	NULL	NULL	0	NULL	special reference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Tracheobronchial clearance in health and disease : with special reference to interciliary fluid .
	manualset3
191494	5	415612	7	NULL	NULL	0	NULL	interciliary fluid 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Tracheobronchial clearance in health and disease : with special reference to interciliary fluid .
	manualset3
191495	1	415613	7	NULL	NULL	NULL	NULL	 hospitalization	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After hospitalization he developed high CRP levels .
	manualset3
191496	2	415613	7	NULL	NULL	0	NULL	high CRP levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After hospitalization he developed high CRP levels .
	manualset3
191497	1	415614	7	NULL	NULL	0	NULL	Tracheostomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Tracheostomy in the paediatric patient has been associated with significant morbidity and mortality compared to that in the adult .
	manualset3
191498	2	415614	7	NULL	NULL	0	NULL	paediatric patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Tracheostomy in the paediatric patient has been associated with significant morbidity and mortality compared to that in the adult .
	manualset3
191499	3	415614	7	NULL	NULL	0	NULL	morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Tracheostomy in the paediatric patient has been associated with significant morbidity and mortality compared to that in the adult .
	manualset3
191500	4	415614	7	NULL	NULL	0	NULL	mortality 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Tracheostomy in the paediatric patient has been associated with significant morbidity and mortality compared to that in the adult .
	manualset3
191501	5	415614	7	NULL	NULL	0	NULL	adult	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Tracheostomy in the paediatric patient has been associated with significant morbidity and mortality compared to that in the adult .
	manualset3
191502	1	415615	7	NULL	NULL	NULL	NULL	trail	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Tracing the trail of protons through complex I of the mitochondrial respiratory chain .
	manualset3
191503	2	415615	7	NULL	NULL	0	NULL	 protons	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Tracing the trail of protons through complex I of the mitochondrial respiratory chain .
	manualset3
191504	3	415615	7	NULL	NULL	0	NULL	complex I	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Tracing the trail of protons through complex I of the mitochondrial respiratory chain .
	manualset3
191505	4	415615	7	NULL	NULL	NULL	NULL	mitochondrial respiratory chain 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Tracing the trail of protons through complex I of the mitochondrial respiratory chain .
	manualset3
193157	5	415615	7	NULL	NULL	NULL	NULL	Tracing	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Tracing the trail of protons through complex I of the mitochondrial respiratory chain .
	manualset3
191506	1	415616	7	NULL	NULL	0	NULL	Traditional blood gas management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditional blood gas management was defined as paO2 values of 150-250 mmHg and average VSAT & lt ; 75 % .
	manualset3
191507	2	415616	7	NULL	NULL	0	NULL	paO2 values 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditional blood gas management was defined as paO2 values of 150-250 mmHg and average VSAT & lt ; 75 % .
	manualset3
191508	3	415616	7	NULL	NULL	0	NULL	150-250 mmHg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditional blood gas management was defined as paO2 values of 150-250 mmHg and average VSAT & lt ; 75 % .
	manualset3
191509	4	415616	7	NULL	NULL	0	NULL	average	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditional blood gas management was defined as paO2 values of 150-250 mmHg and average VSAT & lt ; 75 % .
	manualset3
191510	5	415616	7	NULL	NULL	0	NULL	VSAT & lt	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditional blood gas management was defined as paO2 values of 150-250 mmHg and average VSAT & lt ; 75 % .
	manualset3
191511	6	415616	7	NULL	NULL	0	NULL	75 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditional blood gas management was defined as paO2 values of 150-250 mmHg and average VSAT & lt ; 75 % .
	manualset3
191512	1	415617	7	NULL	NULL	0	NULL	Traditional data-review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditional data-review displays are driven by the ancillary systems that produced the data .
	manualset3
191513	2	415617	7	NULL	NULL	0	NULL	ancillary systems 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditional data-review displays are driven by the ancillary systems that produced the data .
	manualset3
191514	3	415617	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditional data-review displays are driven by the ancillary systems that produced the data .
	manualset3
191515	1	415618	7	NULL	NULL	0	NULL	Traditional measures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditional measures of exposure such as total particulate matter ( TPM ) and benzene soluble matter ( BSM ) were monitored .
	manualset3
191516	2	415618	7	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditional measures of exposure such as total particulate matter ( TPM ) and benzene soluble matter ( BSM ) were monitored .
	manualset3
191517	3	415618	7	NULL	NULL	0	NULL	total particulate matter ( TPM )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditional measures of exposure such as total particulate matter ( TPM ) and benzene soluble matter ( BSM ) were monitored .
	manualset3
191518	4	415618	7	NULL	NULL	0	NULL	benzene soluble matter ( BSM )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditional measures of exposure such as total particulate matter ( TPM ) and benzene soluble matter ( BSM ) were monitored .
	manualset3
191519	1	415619	7	NULL	NULL	0	NULL	Traditional understanding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditional understanding of the baroreceptor system is that inhibition is a result of a blood pressure drop .
	manualset3
191520	2	415619	7	NULL	NULL	0	NULL	baroreceptor system	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditional understanding of the baroreceptor system is that inhibition is a result of a blood pressure drop .
	manualset3
191521	3	415619	7	NULL	NULL	0	NULL	inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditional understanding of the baroreceptor system is that inhibition is a result of a blood pressure drop .
	manualset3
191522	4	415619	7	NULL	NULL	0	NULL	 result	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditional understanding of the baroreceptor system is that inhibition is a result of a blood pressure drop .
	manualset3
191523	5	415619	7	NULL	NULL	0	NULL	blood pressure drop	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditional understanding of the baroreceptor system is that inhibition is a result of a blood pressure drop .
	manualset3
191524	1	415620	7	NULL	NULL	0	NULL	animal models	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , animal models of schizophrenia were predominantly pharmacological constructs focused on phenomena linked to dopamine and glutamate neurotransmitter systems , and were created by direct perturbations of these systems .
	manualset3
191525	2	415620	7	NULL	NULL	0	NULL	schizophrenia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , animal models of schizophrenia were predominantly pharmacological constructs focused on phenomena linked to dopamine and glutamate neurotransmitter systems , and were created by direct perturbations of these systems .
	manualset3
191526	3	415620	7	NULL	NULL	0	NULL	pharmacological constructs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , animal models of schizophrenia were predominantly pharmacological constructs focused on phenomena linked to dopamine and glutamate neurotransmitter systems , and were created by direct perturbations of these systems .
	manualset3
191527	4	415620	7	NULL	NULL	0	NULL	phenomena	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , animal models of schizophrenia were predominantly pharmacological constructs focused on phenomena linked to dopamine and glutamate neurotransmitter systems , and were created by direct perturbations of these systems .
	manualset3
191528	5	415620	7	NULL	NULL	0	NULL	dopamine systems	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , animal models of schizophrenia were predominantly pharmacological constructs focused on phenomena linked to dopamine and glutamate neurotransmitter systems , and were created by direct perturbations of these systems .
	manualset3
191529	6	415620	7	NULL	NULL	0	NULL	glutamate neurotransmitter systems	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , animal models of schizophrenia were predominantly pharmacological constructs focused on phenomena linked to dopamine and glutamate neurotransmitter systems , and were created by direct perturbations of these systems .
	manualset3
191530	7	415620	7	NULL	NULL	0	NULL	direct perturbations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , animal models of schizophrenia were predominantly pharmacological constructs focused on phenomena linked to dopamine and glutamate neurotransmitter systems , and were created by direct perturbations of these systems .
	manualset3
191531	8	415620	7	NULL	NULL	0	NULL	systems	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , animal models of schizophrenia were predominantly pharmacological constructs focused on phenomena linked to dopamine and glutamate neurotransmitter systems , and were created by direct perturbations of these systems .
	manualset3
191532	1	415621	7	NULL	NULL	0	NULL	chromatographic techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , chromatographic techniques such as High Performance Liquid Chromatography ( HPLC ) and Gas Chromatography ( GC ) in conjunction with other analytical techniques have been used to determine the purity and strength of a specific lot of a compound for the purpose of qualifying the lot to use as a reference standard .
	manualset3
191533	2	415621	7	NULL	NULL	0	NULL	High Performance Liquid Chromatography ( HPLC )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , chromatographic techniques such as High Performance Liquid Chromatography ( HPLC ) and Gas Chromatography ( GC ) in conjunction with other analytical techniques have been used to determine the purity and strength of a specific lot of a compound for the purpose of qualifying the lot to use as a reference standard .
	manualset3
191534	3	415621	7	NULL	NULL	0	NULL	Gas Chromatography ( GC )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , chromatographic techniques such as High Performance Liquid Chromatography ( HPLC ) and Gas Chromatography ( GC ) in conjunction with other analytical techniques have been used to determine the purity and strength of a specific lot of a compound for the purpose of qualifying the lot to use as a reference standard .
	manualset3
191535	4	415621	7	NULL	NULL	0	NULL	conjunction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , chromatographic techniques such as High Performance Liquid Chromatography ( HPLC ) and Gas Chromatography ( GC ) in conjunction with other analytical techniques have been used to determine the purity and strength of a specific lot of a compound for the purpose of qualifying the lot to use as a reference standard .
	manualset3
191536	5	415621	7	NULL	NULL	0	NULL	analytical techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , chromatographic techniques such as High Performance Liquid Chromatography ( HPLC ) and Gas Chromatography ( GC ) in conjunction with other analytical techniques have been used to determine the purity and strength of a specific lot of a compound for the purpose of qualifying the lot to use as a reference standard .
	manualset3
191537	6	415621	7	NULL	NULL	0	NULL	purity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , chromatographic techniques such as High Performance Liquid Chromatography ( HPLC ) and Gas Chromatography ( GC ) in conjunction with other analytical techniques have been used to determine the purity and strength of a specific lot of a compound for the purpose of qualifying the lot to use as a reference standard .
	manualset3
191538	7	415621	7	NULL	NULL	0	NULL	strength	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , chromatographic techniques such as High Performance Liquid Chromatography ( HPLC ) and Gas Chromatography ( GC ) in conjunction with other analytical techniques have been used to determine the purity and strength of a specific lot of a compound for the purpose of qualifying the lot to use as a reference standard .
	manualset3
191539	8	415621	7	NULL	NULL	0	NULL	compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , chromatographic techniques such as High Performance Liquid Chromatography ( HPLC ) and Gas Chromatography ( GC ) in conjunction with other analytical techniques have been used to determine the purity and strength of a specific lot of a compound for the purpose of qualifying the lot to use as a reference standard .
	manualset3
191540	9	415621	7	NULL	NULL	0	NULL	purpose 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , chromatographic techniques such as High Performance Liquid Chromatography ( HPLC ) and Gas Chromatography ( GC ) in conjunction with other analytical techniques have been used to determine the purity and strength of a specific lot of a compound for the purpose of qualifying the lot to use as a reference standard .
	manualset3
191541	10	415621	7	NULL	NULL	0	NULL	qualifying 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , chromatographic techniques such as High Performance Liquid Chromatography ( HPLC ) and Gas Chromatography ( GC ) in conjunction with other analytical techniques have been used to determine the purity and strength of a specific lot of a compound for the purpose of qualifying the lot to use as a reference standard .
	manualset3
191542	11	415621	7	NULL	NULL	0	NULL	 lot 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , chromatographic techniques such as High Performance Liquid Chromatography ( HPLC ) and Gas Chromatography ( GC ) in conjunction with other analytical techniques have been used to determine the purity and strength of a specific lot of a compound for the purpose of qualifying the lot to use as a reference standard .
	manualset3
191543	12	415621	7	NULL	NULL	0	NULL	 reference standard	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , chromatographic techniques such as High Performance Liquid Chromatography ( HPLC ) and Gas Chromatography ( GC ) in conjunction with other analytical techniques have been used to determine the purity and strength of a specific lot of a compound for the purpose of qualifying the lot to use as a reference standard .
	manualset3
191544	13	415621	7	NULL	NULL	0	NULL	lot	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , chromatographic techniques such as High Performance Liquid Chromatography ( HPLC ) and Gas Chromatography ( GC ) in conjunction with other analytical techniques have been used to determine the purity and strength of a specific lot of a compound for the purpose of qualifying the lot to use as a reference standard .
	manualset3
191545	1	415622	7	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , exposure to a variety of patients has been achieved through years of training under the supervision of experts in the field .
	manualset3
191546	2	415622	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , exposure to a variety of patients has been achieved through years of training under the supervision of experts in the field .
	manualset3
191547	3	415622	7	NULL	NULL	0	NULL	 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , exposure to a variety of patients has been achieved through years of training under the supervision of experts in the field .
	manualset3
191551	4	415622	7	NULL	NULL	0	NULL	training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , exposure to a variety of patients has been achieved through years of training under the supervision of experts in the field .
	manualset3
191552	5	415622	7	NULL	NULL	0	NULL	supervision	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , exposure to a variety of patients has been achieved through years of training under the supervision of experts in the field .
	manualset3
191553	6	415622	7	NULL	NULL	0	NULL	experts	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , exposure to a variety of patients has been achieved through years of training under the supervision of experts in the field .
	manualset3
191554	7	415622	7	NULL	NULL	NULL	NULL	field	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Traditionally , exposure to a variety of patients has been achieved through years of training under the supervision of experts in the field .
	manualset3
191557	1	415623	7	NULL	NULL	0	NULL	 i.v. dosing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After i.v. dosing , SB-240563 concentration declined in a biexponential manner with a mean terminal half-life of 13 + / - 2 days .
	manualset3
191560	2	415623	7	NULL	NULL	0	NULL	SB-240563 concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After i.v. dosing , SB-240563 concentration declined in a biexponential manner with a mean terminal half-life of 13 + / - 2 days .
	manualset3
191562	3	415623	7	NULL	NULL	0	NULL	biexponential manner	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After i.v. dosing , SB-240563 concentration declined in a biexponential manner with a mean terminal half-life of 13 + / - 2 days .
	manualset3
191564	4	415623	7	NULL	NULL	0	NULL	mean terminal half-life	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After i.v. dosing , SB-240563 concentration declined in a biexponential manner with a mean terminal half-life of 13 + / - 2 days .
	manualset3
191566	5	415623	7	NULL	NULL	0	NULL	13 + / - 2 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After i.v. dosing , SB-240563 concentration declined in a biexponential manner with a mean terminal half-life of 13 + / - 2 days .
	manualset3
191569	1	415624	7	NULL	NULL	0	NULL	lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , these lesions have been made with the radiofrequency technique .
	manualset3
191570	2	415624	7	NULL	NULL	0	NULL	 radiofrequency technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , these lesions have been made with the radiofrequency technique .
	manualset3
191572	1	415625	7	NULL	NULL	0	NULL	tobacco	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , tobacco has been ignored as an issue in the treatment of addictions to alcohol and other drugs .
	manualset3
191574	2	415625	7	NULL	NULL	0	NULL	 issue	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , tobacco has been ignored as an issue in the treatment of addictions to alcohol and other drugs .
	manualset3
191575	3	415625	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , tobacco has been ignored as an issue in the treatment of addictions to alcohol and other drugs .
	manualset3
191578	4	415625	7	NULL	NULL	0	NULL	addictions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , tobacco has been ignored as an issue in the treatment of addictions to alcohol and other drugs .
	manualset3
191580	5	415625	7	NULL	NULL	0	NULL	alcohol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , tobacco has been ignored as an issue in the treatment of addictions to alcohol and other drugs .
	manualset3
191582	6	415625	7	NULL	NULL	0	NULL	 drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , tobacco has been ignored as an issue in the treatment of addictions to alcohol and other drugs .
	manualset3
191583	1	415626	7	NULL	NULL	0	NULL	policymakers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally as well , policymakers have brought the three discrete perspectives of criminology , criminal justice and public health to bear on the problem .
	manualset3
191584	2	415626	7	NULL	NULL	0	NULL	three discrete perspectives	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally as well , policymakers have brought the three discrete perspectives of criminology , criminal justice and public health to bear on the problem .
	manualset3
191585	3	415626	7	NULL	NULL	0	NULL	criminology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally as well , policymakers have brought the three discrete perspectives of criminology , criminal justice and public health to bear on the problem .
	manualset3
191586	4	415626	7	NULL	NULL	0	NULL	criminal justice 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally as well , policymakers have brought the three discrete perspectives of criminology , criminal justice and public health to bear on the problem .
	manualset3
191587	5	415626	7	NULL	NULL	0	NULL	public health 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally as well , policymakers have brought the three discrete perspectives of criminology , criminal justice and public health to bear on the problem .
	manualset3
191588	6	415626	7	NULL	NULL	0	NULL	problem	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally as well , policymakers have brought the three discrete perspectives of criminology , criminal justice and public health to bear on the problem .
	manualset3
191589	1	415627	7	NULL	NULL	0	NULL	Trafficking 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Trafficking of syntaxin1A to the plasma membrane was dependent on the presence of Munc18-1 .
	manualset3
191590	2	415627	7	NULL	NULL	0	NULL	syntaxin1A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Trafficking of syntaxin1A to the plasma membrane was dependent on the presence of Munc18-1 .
	manualset3
191591	3	415627	7	NULL	NULL	0	NULL	plasma membrane 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Trafficking of syntaxin1A to the plasma membrane was dependent on the presence of Munc18-1 .
	manualset3
191592	4	415627	7	NULL	NULL	NULL	NULL	presence	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Trafficking of syntaxin1A to the plasma membrane was dependent on the presence of Munc18-1 .
	manualset3
191593	5	415627	7	NULL	NULL	0	NULL	Munc18-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Trafficking of syntaxin1A to the plasma membrane was dependent on the presence of Munc18-1 .
	manualset3
191594	1	415628	7	NULL	NULL	0	NULL	Training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Training would cover primary health care , community resources , communication and education techniques , and community-based information systems .
	manualset3
191595	2	415628	7	NULL	NULL	0	NULL	primary health care	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Training would cover primary health care , community resources , communication and education techniques , and community-based information systems .
	manualset3
191596	3	415628	7	NULL	NULL	0	NULL	community resources	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Training would cover primary health care , community resources , communication and education techniques , and community-based information systems .
	manualset3
191597	4	415628	7	NULL	NULL	0	NULL	communication techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Training would cover primary health care , community resources , communication and education techniques , and community-based information systems .
	manualset3
191598	5	415628	7	NULL	NULL	0	NULL	education techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Training would cover primary health care , community resources , communication and education techniques , and community-based information systems .
	manualset3
191599	6	415628	7	NULL	NULL	0	NULL	community-based information systems	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Training would cover primary health care , community resources , communication and education techniques , and community-based information systems .
	manualset3
191600	1	415629	7	NULL	NULL	0	NULL	implantation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After implantation , there was a significant increase in total thickness and neointimal hyperplasia with increasing stent force .
	manualset3
191601	2	415629	7	NULL	NULL	0	NULL	increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After implantation , there was a significant increase in total thickness and neointimal hyperplasia with increasing stent force .
	manualset3
191602	3	415629	7	NULL	NULL	0	NULL	total thickness	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After implantation , there was a significant increase in total thickness and neointimal hyperplasia with increasing stent force .
	manualset3
191603	4	415629	7	NULL	NULL	0	NULL	neointimal hyperplasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After implantation , there was a significant increase in total thickness and neointimal hyperplasia with increasing stent force .
	manualset3
191604	5	415629	7	NULL	NULL	0	NULL	stent force 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After implantation , there was a significant increase in total thickness and neointimal hyperplasia with increasing stent force .
	manualset3
191605	1	415630	7	NULL	NULL	NULL	NULL	Trance	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Trance , transference and countertransference in the resistive patient .
	manualset3
191606	2	415630	7	NULL	NULL	0	NULL	 transference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Trance , transference and countertransference in the resistive patient .
	manualset3
191607	3	415630	7	NULL	NULL	0	NULL	countertransference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Trance , transference and countertransference in the resistive patient .
	manualset3
191608	4	415630	7	NULL	NULL	0	NULL	resistive patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Trance , transference and countertransference in the resistive patient .
	manualset3
191776	1	415631	7	NULL	NULL	0	NULL	Trans-resveratrol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Trans-resveratrol added to plasma was distributed between subsequently isolated lipoproteins with a linear dose-response curve .
	manualset3
191777	2	415631	7	NULL	NULL	0	NULL	plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Trans-resveratrol added to plasma was distributed between subsequently isolated lipoproteins with a linear dose-response curve .
	manualset3
191778	3	415631	7	NULL	NULL	0	NULL	isolated lipoproteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Trans-resveratrol added to plasma was distributed between subsequently isolated lipoproteins with a linear dose-response curve .
	manualset3
191779	4	415631	7	NULL	NULL	0	NULL	linear dose-response curve	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Trans-resveratrol added to plasma was distributed between subsequently isolated lipoproteins with a linear dose-response curve .
	manualset3
191781	1	415632	7	NULL	NULL	0	NULL	Trans -- ) cis isomerization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Trans -- ) cis isomerization of N-methylacetylamide ( MeCO-NHMe ) has been studied at the G3MP2B3 level of theory and the vibration spectrum has been calculated as a function of the torsional mode of motion along the peptide bond .
	manualset3
191782	2	415632	7	NULL	NULL	0	NULL	N-methylacetylamide ( MeCO-NHMe )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Trans -- ) cis isomerization of N-methylacetylamide ( MeCO-NHMe ) has been studied at the G3MP2B3 level of theory and the vibration spectrum has been calculated as a function of the torsional mode of motion along the peptide bond .
	manualset3
191784	3	415632	7	NULL	NULL	0	NULL	G3MP2B3 level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Trans -- ) cis isomerization of N-methylacetylamide ( MeCO-NHMe ) has been studied at the G3MP2B3 level of theory and the vibration spectrum has been calculated as a function of the torsional mode of motion along the peptide bond .
	manualset3
191787	4	415632	7	NULL	NULL	0	NULL	theory spectrum	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Trans -- ) cis isomerization of N-methylacetylamide ( MeCO-NHMe ) has been studied at the G3MP2B3 level of theory and the vibration spectrum has been calculated as a function of the torsional mode of motion along the peptide bond .
	manualset3
191789	5	415632	7	NULL	NULL	0	NULL	vibration spectrum	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Trans -- ) cis isomerization of N-methylacetylamide ( MeCO-NHMe ) has been studied at the G3MP2B3 level of theory and the vibration spectrum has been calculated as a function of the torsional mode of motion along the peptide bond .
	manualset3
191790	6	415632	7	NULL	NULL	NULL	NULL	function	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Trans -- ) cis isomerization of N-methylacetylamide ( MeCO-NHMe ) has been studied at the G3MP2B3 level of theory and the vibration spectrum has been calculated as a function of the torsional mode of motion along the peptide bond .
	manualset3
191791	7	415632	7	NULL	NULL	NULL	NULL	torsional mode	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Trans -- ) cis isomerization of N-methylacetylamide ( MeCO-NHMe ) has been studied at the G3MP2B3 level of theory and the vibration spectrum has been calculated as a function of the torsional mode of motion along the peptide bond .
	manualset3
191792	8	415632	7	NULL	NULL	0	NULL	motion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Trans -- ) cis isomerization of N-methylacetylamide ( MeCO-NHMe ) has been studied at the G3MP2B3 level of theory and the vibration spectrum has been calculated as a function of the torsional mode of motion along the peptide bond .
	manualset3
191794	9	415632	7	NULL	NULL	NULL	NULL	peptide bond	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Trans -- ) cis isomerization of N-methylacetylamide ( MeCO-NHMe ) has been studied at the G3MP2B3 level of theory and the vibration spectrum has been calculated as a function of the torsional mode of motion along the peptide bond .
	manualset3
191799	1	415633	7	NULL	NULL	0	NULL	Transabdominal ultrasonography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Transabdominal ultrasonography is frequently used to diagnose small intestinal intussusceptions in foals .
	manualset3
191801	2	415633	7	NULL	NULL	0	NULL	small intestinal intussusceptions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Transabdominal ultrasonography is frequently used to diagnose small intestinal intussusceptions in foals .
	manualset3
191804	3	415633	7	NULL	NULL	0	NULL	foals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Transabdominal ultrasonography is frequently used to diagnose small intestinal intussusceptions in foals .
	manualset3
191808	1	415634	7	NULL	NULL	0	NULL	Transbronchial brachytherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Transbronchial brachytherapy of recurrent bronchogenic carcinoma : a new approach using the flexible fiberoptic bronchoscope .
	manualset3
191811	2	415634	7	NULL	NULL	0	NULL	recurrent bronchogenic carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Transbronchial brachytherapy of recurrent bronchogenic carcinoma : a new approach using the flexible fiberoptic bronchoscope .
	manualset3
191812	3	415634	7	NULL	NULL	0	NULL	new approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transbronchial brachytherapy of recurrent bronchogenic carcinoma : a new approach using the flexible fiberoptic bronchoscope .
	manualset3
191813	4	415634	7	NULL	NULL	0	NULL	flexible fiberoptic bronchoscope	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Transbronchial brachytherapy of recurrent bronchogenic carcinoma : a new approach using the flexible fiberoptic bronchoscope .
	manualset3
191814	1	415635	7	NULL	NULL	0	NULL	Transcranial magnetic stimulation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcranial magnetic stimulation or repetitive transcranial magnetic stimulation ( TMS/rTMS ) is currently being used in treatments of the central nervous system diseases , for instance , depressive states .
	manualset3
191815	2	415635	7	NULL	NULL	0	NULL	repetitive transcranial magnetic stimulation ( TMS/rTMS )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcranial magnetic stimulation or repetitive transcranial magnetic stimulation ( TMS/rTMS ) is currently being used in treatments of the central nervous system diseases , for instance , depressive states .
	manualset3
191816	3	415635	7	NULL	NULL	0	NULL	treatments	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcranial magnetic stimulation or repetitive transcranial magnetic stimulation ( TMS/rTMS ) is currently being used in treatments of the central nervous system diseases , for instance , depressive states .
	manualset3
191817	4	415635	7	NULL	NULL	0	NULL	central nervous system diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcranial magnetic stimulation or repetitive transcranial magnetic stimulation ( TMS/rTMS ) is currently being used in treatments of the central nervous system diseases , for instance , depressive states .
	manualset3
191818	5	415635	7	NULL	NULL	0	NULL	depressive states	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcranial magnetic stimulation or repetitive transcranial magnetic stimulation ( TMS/rTMS ) is currently being used in treatments of the central nervous system diseases , for instance , depressive states .
	manualset3
191819	1	415636	7	NULL	NULL	0	NULL	Transcript mapping 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcript mapping and processing of mitochondrial RNA in the chlorophyte alga Prototheca wickerhamii .
	manualset3
191820	2	415636	7	NULL	NULL	0	NULL	processing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcript mapping and processing of mitochondrial RNA in the chlorophyte alga Prototheca wickerhamii .
	manualset3
191821	3	415636	7	NULL	NULL	0	NULL	mitochondrial RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcript mapping and processing of mitochondrial RNA in the chlorophyte alga Prototheca wickerhamii .
	manualset3
191822	4	415636	7	NULL	NULL	0	NULL	chlorophyte alga Prototheca wickerhamii 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcript mapping and processing of mitochondrial RNA in the chlorophyte alga Prototheca wickerhamii .
	manualset3
191823	1	415637	7	NULL	NULL	0	NULL	Transcriptional regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcriptional regulation of multidrug efflux pumps in bacteria .
	manualset3
191824	2	415637	7	NULL	NULL	0	NULL	multidrug efflux pumps	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcriptional regulation of multidrug efflux pumps in bacteria .
	manualset3
191825	3	415637	7	NULL	NULL	0	NULL	bacteria 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcriptional regulation of multidrug efflux pumps in bacteria .
	manualset3
191826	1	415638	7	NULL	NULL	0	NULL	Transcripts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcripts of the three maize Enhancer of zeste-like genes , Mez1 , Mez2 , and Mez3 , were detected in all tissues tested , and the Mez2 transcript is alternatively spliced in a tissue-dependent pattern .
	manualset3
191827	2	415638	7	NULL	NULL	0	NULL	three maize Enhancer of zeste-like genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcripts of the three maize Enhancer of zeste-like genes , Mez1 , Mez2 , and Mez3 , were detected in all tissues tested , and the Mez2 transcript is alternatively spliced in a tissue-dependent pattern .
	manualset3
191828	3	415638	7	NULL	NULL	0	NULL	Mez1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcripts of the three maize Enhancer of zeste-like genes , Mez1 , Mez2 , and Mez3 , were detected in all tissues tested , and the Mez2 transcript is alternatively spliced in a tissue-dependent pattern .
	manualset3
191829	4	415638	7	NULL	NULL	0	NULL	Mez2	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcripts of the three maize Enhancer of zeste-like genes , Mez1 , Mez2 , and Mez3 , were detected in all tissues tested , and the Mez2 transcript is alternatively spliced in a tissue-dependent pattern .
	manualset3
191830	5	415638	7	NULL	NULL	0	NULL	Mez3	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcripts of the three maize Enhancer of zeste-like genes , Mez1 , Mez2 , and Mez3 , were detected in all tissues tested , and the Mez2 transcript is alternatively spliced in a tissue-dependent pattern .
	manualset3
191831	6	415638	7	NULL	NULL	0	NULL	tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcripts of the three maize Enhancer of zeste-like genes , Mez1 , Mez2 , and Mez3 , were detected in all tissues tested , and the Mez2 transcript is alternatively spliced in a tissue-dependent pattern .
	manualset3
191832	7	415638	7	NULL	NULL	0	NULL	Mez2 transcript	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcripts of the three maize Enhancer of zeste-like genes , Mez1 , Mez2 , and Mez3 , were detected in all tissues tested , and the Mez2 transcript is alternatively spliced in a tissue-dependent pattern .
	manualset3
191833	8	415638	7	NULL	NULL	0	NULL	tissue-dependent pattern	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcripts of the three maize Enhancer of zeste-like genes , Mez1 , Mez2 , and Mez3 , were detected in all tissues tested , and the Mez2 transcript is alternatively spliced in a tissue-dependent pattern .
	manualset3
191834	1	415639	7	NULL	NULL	0	NULL	Transcutaneous color Doppler sonography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcutaneous color Doppler sonography of lung consolidations : review and pictorial essay .
	manualset3
191835	2	415639	7	NULL	NULL	0	NULL	 lung consolidations 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcutaneous color Doppler sonography of lung consolidations : review and pictorial essay .
	manualset3
191836	3	415639	7	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcutaneous color Doppler sonography of lung consolidations : review and pictorial essay .
	manualset3
191837	4	415639	7	NULL	NULL	0	NULL	pictorial essay	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcutaneous color Doppler sonography of lung consolidations : review and pictorial essay .
	manualset3
191840	1	415640	7	NULL	NULL	0	NULL	Transcytosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcytosis of dIgA was not due to paracellular leakage and was inhibited to approximately 20 and 30 % of control values by anti-pIgR antibodies and the competitive ligand pentameric IgM , respectively .
	manualset3
191843	2	415640	7	NULL	NULL	0	NULL	dIgA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcytosis of dIgA was not due to paracellular leakage and was inhibited to approximately 20 and 30 % of control values by anti-pIgR antibodies and the competitive ligand pentameric IgM , respectively .
	manualset3
191845	3	415640	7	NULL	NULL	0	NULL	paracellular leakage 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcytosis of dIgA was not due to paracellular leakage and was inhibited to approximately 20 and 30 % of control values by anti-pIgR antibodies and the competitive ligand pentameric IgM , respectively .
	manualset3
191846	4	415640	7	NULL	NULL	0	NULL	20%	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcytosis of dIgA was not due to paracellular leakage and was inhibited to approximately 20 and 30 % of control values by anti-pIgR antibodies and the competitive ligand pentameric IgM , respectively .
	manualset3
191847	5	415640	7	NULL	NULL	0	NULL	30 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcytosis of dIgA was not due to paracellular leakage and was inhibited to approximately 20 and 30 % of control values by anti-pIgR antibodies and the competitive ligand pentameric IgM , respectively .
	manualset3
191848	6	415640	7	NULL	NULL	0	NULL	control values 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcytosis of dIgA was not due to paracellular leakage and was inhibited to approximately 20 and 30 % of control values by anti-pIgR antibodies and the competitive ligand pentameric IgM , respectively .
	manualset3
191849	7	415640	7	NULL	NULL	0	NULL	anti-pIgR antibodies 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcytosis of dIgA was not due to paracellular leakage and was inhibited to approximately 20 and 30 % of control values by anti-pIgR antibodies and the competitive ligand pentameric IgM , respectively .
	manualset3
191850	8	415640	7	NULL	NULL	0	NULL	competitive ligand pentameric IgM 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcytosis of dIgA was not due to paracellular leakage and was inhibited to approximately 20 and 30 % of control values by anti-pIgR antibodies and the competitive ligand pentameric IgM , respectively .
	manualset3
192079	1	415641	7	NULL	NULL	0	NULL	Transepithelial short-circuit current ( I ( sc ) )	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Transepithelial short-circuit current ( I ( sc ) ) and transepithelial conductance ( G ( t ) ) were measured for colonic mucosa during secretory activation by epinephrine ( EPI ) , prostaglandin E ( 2 ) ( PGE ( 2 ) ) , and carbachol ( CCh ) .
	manualset3
192080	2	415641	7	NULL	NULL	0	NULL	transepithelial conductance ( G ( t ) )	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Transepithelial short-circuit current ( I ( sc ) ) and transepithelial conductance ( G ( t ) ) were measured for colonic mucosa during secretory activation by epinephrine ( EPI ) , prostaglandin E ( 2 ) ( PGE ( 2 ) ) , and carbachol ( CCh ) .
	manualset3
192081	3	415641	7	NULL	NULL	0	NULL	colonic mucosa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Transepithelial short-circuit current ( I ( sc ) ) and transepithelial conductance ( G ( t ) ) were measured for colonic mucosa during secretory activation by epinephrine ( EPI ) , prostaglandin E ( 2 ) ( PGE ( 2 ) ) , and carbachol ( CCh ) .
	manualset3
192082	4	415641	7	NULL	NULL	0	NULL	secretory activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transepithelial short-circuit current ( I ( sc ) ) and transepithelial conductance ( G ( t ) ) were measured for colonic mucosa during secretory activation by epinephrine ( EPI ) , prostaglandin E ( 2 ) ( PGE ( 2 ) ) , and carbachol ( CCh ) .
	manualset3
192083	5	415641	7	NULL	NULL	0	NULL	epinephrine ( EPI )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Transepithelial short-circuit current ( I ( sc ) ) and transepithelial conductance ( G ( t ) ) were measured for colonic mucosa during secretory activation by epinephrine ( EPI ) , prostaglandin E ( 2 ) ( PGE ( 2 ) ) , and carbachol ( CCh ) .
	manualset3
192084	6	415641	7	NULL	NULL	0	NULL	prostaglandin E ( 2 )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Transepithelial short-circuit current ( I ( sc ) ) and transepithelial conductance ( G ( t ) ) were measured for colonic mucosa during secretory activation by epinephrine ( EPI ) , prostaglandin E ( 2 ) ( PGE ( 2 ) ) , and carbachol ( CCh ) .
	manualset3
192085	7	415641	7	NULL	NULL	0	NULL	( PGE ( 2 ) )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Transepithelial short-circuit current ( I ( sc ) ) and transepithelial conductance ( G ( t ) ) were measured for colonic mucosa during secretory activation by epinephrine ( EPI ) , prostaglandin E ( 2 ) ( PGE ( 2 ) ) , and carbachol ( CCh ) .
	manualset3
192086	8	415641	7	NULL	NULL	0	NULL	carbachol ( CCh )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Transepithelial short-circuit current ( I ( sc ) ) and transepithelial conductance ( G ( t ) ) were measured for colonic mucosa during secretory activation by epinephrine ( EPI ) , prostaglandin E ( 2 ) ( PGE ( 2 ) ) , and carbachol ( CCh ) .
	manualset3
192087	1	415642	7	NULL	NULL	0	NULL	Transepithelial transport	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transepithelial transport of alpha-mangostin was increased during prandial-like compared to fasted conditions suggesting that absorption is enhanced by dietary fat .
	manualset3
192088	2	415642	7	NULL	NULL	NULL	NULL	alpha-mangostin	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Transepithelial transport of alpha-mangostin was increased during prandial-like compared to fasted conditions suggesting that absorption is enhanced by dietary fat .
	manualset3
192089	3	415642	7	NULL	NULL	0	NULL	prandial-like conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Transepithelial transport of alpha-mangostin was increased during prandial-like compared to fasted conditions suggesting that absorption is enhanced by dietary fat .
	manualset3
192090	4	415642	7	NULL	NULL	0	NULL	fasted conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Transepithelial transport of alpha-mangostin was increased during prandial-like compared to fasted conditions suggesting that absorption is enhanced by dietary fat .
	manualset3
192091	5	415642	7	NULL	NULL	0	NULL	absorption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transepithelial transport of alpha-mangostin was increased during prandial-like compared to fasted conditions suggesting that absorption is enhanced by dietary fat .
	manualset3
192092	6	415642	7	NULL	NULL	0	NULL	 dietary fat	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Transepithelial transport of alpha-mangostin was increased during prandial-like compared to fasted conditions suggesting that absorption is enhanced by dietary fat .
	manualset3
192093	1	415643	7	NULL	NULL	0	NULL	Transfected cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfected cells expressing Us5/gJ were also protected from death induced by incubation with purified grB and perforin .
	manualset3
192094	2	415643	7	NULL	NULL	0	NULL	 Us5/gJ	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfected cells expressing Us5/gJ were also protected from death induced by incubation with purified grB and perforin .
	manualset3
192095	3	415643	7	NULL	NULL	0	NULL	death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfected cells expressing Us5/gJ were also protected from death induced by incubation with purified grB and perforin .
	manualset3
192096	4	415643	7	NULL	NULL	0	NULL	incubation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfected cells expressing Us5/gJ were also protected from death induced by incubation with purified grB and perforin .
	manualset3
192097	5	415643	7	NULL	NULL	0	NULL	 purified grB 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfected cells expressing Us5/gJ were also protected from death induced by incubation with purified grB and perforin .
	manualset3
192098	6	415643	7	NULL	NULL	0	NULL	perforin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfected cells expressing Us5/gJ were also protected from death induced by incubation with purified grB and perforin .
	manualset3
192099	1	415644	7	NULL	NULL	0	NULL	Transfection assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfection assays with a luciferase reporter gene revealed that cell-specific expression in vitro was retained in a 292 bp sequence , which contained several consensus binding motifs for transcriptional factors preferentially expressed in cells of the lymphoid lineages .
	manualset3
192100	2	415644	7	NULL	NULL	0	NULL	luciferase reporter gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfection assays with a luciferase reporter gene revealed that cell-specific expression in vitro was retained in a 292 bp sequence , which contained several consensus binding motifs for transcriptional factors preferentially expressed in cells of the lymphoid lineages .
	manualset3
192101	3	415644	7	NULL	NULL	NULL	NULL	cell-specific expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Transfection assays with a luciferase reporter gene revealed that cell-specific expression in vitro was retained in a 292 bp sequence , which contained several consensus binding motifs for transcriptional factors preferentially expressed in cells of the lymphoid lineages .
	manualset3
192102	4	415644	7	NULL	NULL	0	NULL	292 bp sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfection assays with a luciferase reporter gene revealed that cell-specific expression in vitro was retained in a 292 bp sequence , which contained several consensus binding motifs for transcriptional factors preferentially expressed in cells of the lymphoid lineages .
	manualset3
192103	5	415644	7	NULL	NULL	0	NULL	several consensus binding motifs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfection assays with a luciferase reporter gene revealed that cell-specific expression in vitro was retained in a 292 bp sequence , which contained several consensus binding motifs for transcriptional factors preferentially expressed in cells of the lymphoid lineages .
	manualset3
192104	6	415644	7	NULL	NULL	0	NULL	transcriptional factors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfection assays with a luciferase reporter gene revealed that cell-specific expression in vitro was retained in a 292 bp sequence , which contained several consensus binding motifs for transcriptional factors preferentially expressed in cells of the lymphoid lineages .
	manualset3
192105	7	415644	7	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfection assays with a luciferase reporter gene revealed that cell-specific expression in vitro was retained in a 292 bp sequence , which contained several consensus binding motifs for transcriptional factors preferentially expressed in cells of the lymphoid lineages .
	manualset3
192106	8	415644	7	NULL	NULL	0	NULL	 lymphoid lineages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfection assays with a luciferase reporter gene revealed that cell-specific expression in vitro was retained in a 292 bp sequence , which contained several consensus binding motifs for transcriptional factors preferentially expressed in cells of the lymphoid lineages .
	manualset3
192146	1	415645	7	NULL	NULL	0	NULL	Transfection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfection efficacies obtained using magnetofection methods were highly competitive with or better than current widely used nonviral transfection methods ( e.g. , electroporation and lipofection ) with the additional critical advantage of high cell viability .
	manualset3
192147	2	415645	7	NULL	NULL	0	NULL	magnetofection methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfection efficacies obtained using magnetofection methods were highly competitive with or better than current widely used nonviral transfection methods ( e.g. , electroporation and lipofection ) with the additional critical advantage of high cell viability .
	manualset3
192148	3	415645	7	NULL	NULL	0	NULL	nonviral transfection methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfection efficacies obtained using magnetofection methods were highly competitive with or better than current widely used nonviral transfection methods ( e.g. , electroporation and lipofection ) with the additional critical advantage of high cell viability .
	manualset3
192149	4	415645	7	NULL	NULL	0	NULL	electroporation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfection efficacies obtained using magnetofection methods were highly competitive with or better than current widely used nonviral transfection methods ( e.g. , electroporation and lipofection ) with the additional critical advantage of high cell viability .
	manualset3
192150	5	415645	7	NULL	NULL	0	NULL	lipofection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfection efficacies obtained using magnetofection methods were highly competitive with or better than current widely used nonviral transfection methods ( e.g. , electroporation and lipofection ) with the additional critical advantage of high cell viability .
	manualset3
192151	6	415645	7	NULL	NULL	NULL	NULL	advantage	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Transfection efficacies obtained using magnetofection methods were highly competitive with or better than current widely used nonviral transfection methods ( e.g. , electroporation and lipofection ) with the additional critical advantage of high cell viability .
	manualset3
192152	7	415645	7	NULL	NULL	0	NULL	high cell viability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfection efficacies obtained using magnetofection methods were highly competitive with or better than current widely used nonviral transfection methods ( e.g. , electroporation and lipofection ) with the additional critical advantage of high cell viability .
	manualset3
192153	1	415646	7	NULL	NULL	NULL	NULL	in vitro digestion	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After in vitro digestion the level of detectable phenolic compounds ( expressed as gallic acid equivalent ) was higher in both pineapple and red fruits juices enriched with Pycnogenol than in non-enriched commercial juices ( 155.6 mg/100mL vs 94.6 mg/100mL and 478.5 mg/100mL vs 406.9 mg/100mL , respectively ) .
	manualset3
192154	2	415646	7	NULL	NULL	0	NULL	 level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After in vitro digestion the level of detectable phenolic compounds ( expressed as gallic acid equivalent ) was higher in both pineapple and red fruits juices enriched with Pycnogenol than in non-enriched commercial juices ( 155.6 mg/100mL vs 94.6 mg/100mL and 478.5 mg/100mL vs 406.9 mg/100mL , respectively ) .
	manualset3
192155	3	415646	7	NULL	NULL	0	NULL	detectable phenolic compounds 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After in vitro digestion the level of detectable phenolic compounds ( expressed as gallic acid equivalent ) was higher in both pineapple and red fruits juices enriched with Pycnogenol than in non-enriched commercial juices ( 155.6 mg/100mL vs 94.6 mg/100mL and 478.5 mg/100mL vs 406.9 mg/100mL , respectively ) .
	manualset3
192156	4	415646	7	NULL	NULL	0	NULL	gallic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After in vitro digestion the level of detectable phenolic compounds ( expressed as gallic acid equivalent ) was higher in both pineapple and red fruits juices enriched with Pycnogenol than in non-enriched commercial juices ( 155.6 mg/100mL vs 94.6 mg/100mL and 478.5 mg/100mL vs 406.9 mg/100mL , respectively ) .
	manualset3
192157	5	415646	7	NULL	NULL	NULL	NULL	pineapple juice	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After in vitro digestion the level of detectable phenolic compounds ( expressed as gallic acid equivalent ) was higher in both pineapple and red fruits juices enriched with Pycnogenol than in non-enriched commercial juices ( 155.6 mg/100mL vs 94.6 mg/100mL and 478.5 mg/100mL vs 406.9 mg/100mL , respectively ) .
	manualset3
192158	6	415646	7	NULL	NULL	NULL	NULL	red fruits juices	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After in vitro digestion the level of detectable phenolic compounds ( expressed as gallic acid equivalent ) was higher in both pineapple and red fruits juices enriched with Pycnogenol than in non-enriched commercial juices ( 155.6 mg/100mL vs 94.6 mg/100mL and 478.5 mg/100mL vs 406.9 mg/100mL , respectively ) .
	manualset3
192159	7	415646	7	NULL	NULL	0	NULL	Pycnogenol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After in vitro digestion the level of detectable phenolic compounds ( expressed as gallic acid equivalent ) was higher in both pineapple and red fruits juices enriched with Pycnogenol than in non-enriched commercial juices ( 155.6 mg/100mL vs 94.6 mg/100mL and 478.5 mg/100mL vs 406.9 mg/100mL , respectively ) .
	manualset3
192160	8	415646	7	NULL	NULL	0	NULL	non-enriched commercial juices 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	After in vitro digestion the level of detectable phenolic compounds ( expressed as gallic acid equivalent ) was higher in both pineapple and red fruits juices enriched with Pycnogenol than in non-enriched commercial juices ( 155.6 mg/100mL vs 94.6 mg/100mL and 478.5 mg/100mL vs 406.9 mg/100mL , respectively ) .
	manualset3
192161	9	415646	7	NULL	NULL	0	NULL	155.6 mg/100mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	After in vitro digestion the level of detectable phenolic compounds ( expressed as gallic acid equivalent ) was higher in both pineapple and red fruits juices enriched with Pycnogenol than in non-enriched commercial juices ( 155.6 mg/100mL vs 94.6 mg/100mL and 478.5 mg/100mL vs 406.9 mg/100mL , respectively ) .
	manualset3
192162	10	415646	7	NULL	NULL	0	NULL	94.6 mg/100mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	After in vitro digestion the level of detectable phenolic compounds ( expressed as gallic acid equivalent ) was higher in both pineapple and red fruits juices enriched with Pycnogenol than in non-enriched commercial juices ( 155.6 mg/100mL vs 94.6 mg/100mL and 478.5 mg/100mL vs 406.9 mg/100mL , respectively ) .
	manualset3
192163	11	415646	7	NULL	NULL	0	NULL	478.5 mg/100mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	After in vitro digestion the level of detectable phenolic compounds ( expressed as gallic acid equivalent ) was higher in both pineapple and red fruits juices enriched with Pycnogenol than in non-enriched commercial juices ( 155.6 mg/100mL vs 94.6 mg/100mL and 478.5 mg/100mL vs 406.9 mg/100mL , respectively ) .
	manualset3
192164	12	415646	7	NULL	NULL	0	NULL	406.9 mg/100mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	After in vitro digestion the level of detectable phenolic compounds ( expressed as gallic acid equivalent ) was higher in both pineapple and red fruits juices enriched with Pycnogenol than in non-enriched commercial juices ( 155.6 mg/100mL vs 94.6 mg/100mL and 478.5 mg/100mL vs 406.9 mg/100mL , respectively ) .
	manualset3
192165	1	415647	7	NULL	NULL	0	NULL	Transfection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfection of TRVb cells or the derivative line TRVb1 ( which stably expresses human TfR1 ) with HFE resulted in lower ferritin levels and decreased Fe2 + uptake .
	manualset3
192166	2	415647	7	NULL	NULL	0	NULL	TRVb cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfection of TRVb cells or the derivative line TRVb1 ( which stably expresses human TfR1 ) with HFE resulted in lower ferritin levels and decreased Fe2 + uptake .
	manualset3
192167	3	415647	7	NULL	NULL	0	NULL	derivative line TRVb1	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfection of TRVb cells or the derivative line TRVb1 ( which stably expresses human TfR1 ) with HFE resulted in lower ferritin levels and decreased Fe2 + uptake .
	manualset3
192168	4	415647	7	NULL	NULL	0	NULL	human TfR1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfection of TRVb cells or the derivative line TRVb1 ( which stably expresses human TfR1 ) with HFE resulted in lower ferritin levels and decreased Fe2 + uptake .
	manualset3
192169	5	415647	7	NULL	NULL	0	NULL	HFE 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfection of TRVb cells or the derivative line TRVb1 ( which stably expresses human TfR1 ) with HFE resulted in lower ferritin levels and decreased Fe2 + uptake .
	manualset3
192170	6	415647	7	NULL	NULL	0	NULL	lower ferritin levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfection of TRVb cells or the derivative line TRVb1 ( which stably expresses human TfR1 ) with HFE resulted in lower ferritin levels and decreased Fe2 + uptake .
	manualset3
192171	7	415647	7	NULL	NULL	0	NULL	Fe2 + uptake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfection of TRVb cells or the derivative line TRVb1 ( which stably expresses human TfR1 ) with HFE resulted in lower ferritin levels and decreased Fe2 + uptake .
	manualset3
192172	1	415648	7	NULL	NULL	0	NULL	Transfer	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfer of fusion colonies from crosses performed in the absence of HU to V8 + HU revealed enhanced hyphal growth in the presence of HU .
	manualset3
192173	2	415648	7	NULL	NULL	0	NULL	fusion colonies	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfer of fusion colonies from crosses performed in the absence of HU to V8 + HU revealed enhanced hyphal growth in the presence of HU .
	manualset3
192174	3	415648	7	NULL	NULL	0	NULL	crosses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfer of fusion colonies from crosses performed in the absence of HU to V8 + HU revealed enhanced hyphal growth in the presence of HU .
	manualset3
192192	4	415648	7	NULL	NULL	0	NULL	HU	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfer of fusion colonies from crosses performed in the absence of HU to V8 + HU revealed enhanced hyphal growth in the presence of HU .
	manualset3
192193	5	415648	7	NULL	NULL	0	NULL	V8 + HU	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfer of fusion colonies from crosses performed in the absence of HU to V8 + HU revealed enhanced hyphal growth in the presence of HU .
	manualset3
192196	6	415648	7	NULL	NULL	0	NULL	enhanced hyphal growth	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfer of fusion colonies from crosses performed in the absence of HU to V8 + HU revealed enhanced hyphal growth in the presence of HU .
	manualset3
192197	7	415648	7	NULL	NULL	0	NULL	 presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfer of fusion colonies from crosses performed in the absence of HU to V8 + HU revealed enhanced hyphal growth in the presence of HU .
	manualset3
192198	8	415648	7	NULL	NULL	0	NULL	HU	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfer of fusion colonies from crosses performed in the absence of HU to V8 + HU revealed enhanced hyphal growth in the presence of HU .
	manualset3
192199	1	415649	7	NULL	NULL	0	NULL	Transfer 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfer of protozoa between ancestors of modern Cryptocercus and termites remains a valid alternative theory to the established hypothesis of symbiont inheritance from a common ancestor .
	manualset3
192200	2	415649	7	NULL	NULL	0	NULL	protozoa	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfer of protozoa between ancestors of modern Cryptocercus and termites remains a valid alternative theory to the established hypothesis of symbiont inheritance from a common ancestor .
	manualset3
192201	3	415649	7	NULL	NULL	0	NULL	ancestors	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfer of protozoa between ancestors of modern Cryptocercus and termites remains a valid alternative theory to the established hypothesis of symbiont inheritance from a common ancestor .
	manualset3
192202	4	415649	7	NULL	NULL	0	NULL	modern Cryptocercus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfer of protozoa between ancestors of modern Cryptocercus and termites remains a valid alternative theory to the established hypothesis of symbiont inheritance from a common ancestor .
	manualset3
192203	5	415649	7	NULL	NULL	0	NULL	termites	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfer of protozoa between ancestors of modern Cryptocercus and termites remains a valid alternative theory to the established hypothesis of symbiont inheritance from a common ancestor .
	manualset3
192204	6	415649	7	NULL	NULL	0	NULL	alternative theory 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfer of protozoa between ancestors of modern Cryptocercus and termites remains a valid alternative theory to the established hypothesis of symbiont inheritance from a common ancestor .
	manualset3
192205	7	415649	7	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfer of protozoa between ancestors of modern Cryptocercus and termites remains a valid alternative theory to the established hypothesis of symbiont inheritance from a common ancestor .
	manualset3
192206	8	415649	7	NULL	NULL	0	NULL	symbiont inheritance	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfer of protozoa between ancestors of modern Cryptocercus and termites remains a valid alternative theory to the established hypothesis of symbiont inheritance from a common ancestor .
	manualset3
192207	9	415649	7	NULL	NULL	0	NULL	common ancestor 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfer of protozoa between ancestors of modern Cryptocercus and termites remains a valid alternative theory to the established hypothesis of symbiont inheritance from a common ancestor .
	manualset3
192208	1	415650	7	NULL	NULL	0	NULL	Transfer	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfer of the wild-type p53 gene using a retrovirus vector to cancer tissues with mutant p53 gene has already been tested clinically .
	manualset3
192209	2	415650	7	NULL	NULL	0	NULL	wild-type p53 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfer of the wild-type p53 gene using a retrovirus vector to cancer tissues with mutant p53 gene has already been tested clinically .
	manualset3
192210	3	415650	7	NULL	NULL	0	NULL	retrovirus vector	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfer of the wild-type p53 gene using a retrovirus vector to cancer tissues with mutant p53 gene has already been tested clinically .
	manualset3
192211	4	415650	7	NULL	NULL	0	NULL	cancer tissues 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfer of the wild-type p53 gene using a retrovirus vector to cancer tissues with mutant p53 gene has already been tested clinically .
	manualset3
192212	5	415650	7	NULL	NULL	0	NULL	mutant p53 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfer of the wild-type p53 gene using a retrovirus vector to cancer tissues with mutant p53 gene has already been tested clinically .
	manualset3
192213	1	415651	7	NULL	NULL	0	NULL	Transfer region	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfer region of pO113 from enterohemorrhagic Escherichia coli : similarity with R64 and identification of a novel plasmid-encoded autotransporter , EpeA .
	manualset3
192214	2	415651	7	NULL	NULL	0	NULL	 pO113	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfer region of pO113 from enterohemorrhagic Escherichia coli : similarity with R64 and identification of a novel plasmid-encoded autotransporter , EpeA .
	manualset3
192215	3	415651	7	NULL	NULL	0	NULL	enterohemorrhagic Escherichia coli 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfer region of pO113 from enterohemorrhagic Escherichia coli : similarity with R64 and identification of a novel plasmid-encoded autotransporter , EpeA .
	manualset3
192216	4	415651	7	NULL	NULL	0	NULL	similarity	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfer region of pO113 from enterohemorrhagic Escherichia coli : similarity with R64 and identification of a novel plasmid-encoded autotransporter , EpeA .
	manualset3
192217	5	415651	7	NULL	NULL	0	NULL	R64	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfer region of pO113 from enterohemorrhagic Escherichia coli : similarity with R64 and identification of a novel plasmid-encoded autotransporter , EpeA .
	manualset3
192218	6	415651	7	NULL	NULL	0	NULL	 identification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfer region of pO113 from enterohemorrhagic Escherichia coli : similarity with R64 and identification of a novel plasmid-encoded autotransporter , EpeA .
	manualset3
192219	7	415651	7	NULL	NULL	0	NULL	novel plasmid-encoded autotransporter ,	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfer region of pO113 from enterohemorrhagic Escherichia coli : similarity with R64 and identification of a novel plasmid-encoded autotransporter , EpeA .
	manualset3
192220	8	415651	7	NULL	NULL	0	NULL	EpeA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Transfer region of pO113 from enterohemorrhagic Escherichia coli : similarity with R64 and identification of a novel plasmid-encoded autotransporter , EpeA .
	manualset3
192221	1	415652	7	NULL	NULL	0	NULL	Transformed cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Transformed cells overexpress a cytosolic nucleic acid binding protein .
	manualset3
192222	2	415652	7	NULL	NULL	0	NULL	cytosolic nucleic acid binding protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Transformed cells overexpress a cytosolic nucleic acid binding protein .
	manualset3
192223	1	415653	7	NULL	NULL	0	NULL	Transforming growth factor-beta induced gene-h3 ( betaig-h3 ) 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Transforming growth factor-beta induced gene-h3 ( betaig-h3 ) was found to co-purify with collagen VI microfibrils , extracted from developing fetal ligament , after equilibrium density gradient centrifugation under both nondenaturing and denaturing conditions .
	manualset3
192224	2	415653	7	NULL	NULL	0	NULL	collagen VI microfibrils	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Transforming growth factor-beta induced gene-h3 ( betaig-h3 ) was found to co-purify with collagen VI microfibrils , extracted from developing fetal ligament , after equilibrium density gradient centrifugation under both nondenaturing and denaturing conditions .
	manualset3
192225	3	415653	7	NULL	NULL	0	NULL	developing fetal ligament 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Transforming growth factor-beta induced gene-h3 ( betaig-h3 ) was found to co-purify with collagen VI microfibrils , extracted from developing fetal ligament , after equilibrium density gradient centrifugation under both nondenaturing and denaturing conditions .
	manualset3
192226	4	415653	7	NULL	NULL	0	NULL	equilibrium density gradient centrifugation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transforming growth factor-beta induced gene-h3 ( betaig-h3 ) was found to co-purify with collagen VI microfibrils , extracted from developing fetal ligament , after equilibrium density gradient centrifugation under both nondenaturing and denaturing conditions .
	manualset3
192227	5	415653	7	NULL	NULL	0	NULL	nondenaturing conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Transforming growth factor-beta induced gene-h3 ( betaig-h3 ) was found to co-purify with collagen VI microfibrils , extracted from developing fetal ligament , after equilibrium density gradient centrifugation under both nondenaturing and denaturing conditions .
	manualset3
192228	6	415653	7	NULL	NULL	0	NULL	denaturing conditions 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Transforming growth factor-beta induced gene-h3 ( betaig-h3 ) was found to co-purify with collagen VI microfibrils , extracted from developing fetal ligament , after equilibrium density gradient centrifugation under both nondenaturing and denaturing conditions .
	manualset3
192229	1	415654	7	NULL	NULL	0	NULL	Transforming growth factor-beta signaling 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transforming growth factor-beta signaling helps specify tumor type in DMBA and hormone-induced mammary cancers .
	manualset3
192230	2	415654	7	NULL	NULL	0	NULL	tumor type	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Transforming growth factor-beta signaling helps specify tumor type in DMBA and hormone-induced mammary cancers .
	manualset3
192231	3	415654	7	NULL	NULL	0	NULL	DMBA mammary cancers	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Transforming growth factor-beta signaling helps specify tumor type in DMBA and hormone-induced mammary cancers .
	manualset3
192232	4	415654	7	NULL	NULL	0	NULL	hormone-induced mammary cancers	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Transforming growth factor-beta signaling helps specify tumor type in DMBA and hormone-induced mammary cancers .
	manualset3
192233	1	415655	7	NULL	NULL	0	NULL	Transforming growth factor - ( TGF - ) signaling	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transforming growth factor - ( TGF - ) signaling is implicated in the pathogenesis of fibrosis in scleroderma or systemic sclerosis ( SSc ) , but the precise mechanisms are poorly understood .
	manualset3
192234	2	415655	7	NULL	NULL	0	NULL	pathogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transforming growth factor - ( TGF - ) signaling is implicated in the pathogenesis of fibrosis in scleroderma or systemic sclerosis ( SSc ) , but the precise mechanisms are poorly understood .
	manualset3
192235	3	415655	7	NULL	NULL	0	NULL	fibrosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Transforming growth factor - ( TGF - ) signaling is implicated in the pathogenesis of fibrosis in scleroderma or systemic sclerosis ( SSc ) , but the precise mechanisms are poorly understood .
	manualset3
192236	4	415655	7	NULL	NULL	0	NULL	scleroderma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Transforming growth factor - ( TGF - ) signaling is implicated in the pathogenesis of fibrosis in scleroderma or systemic sclerosis ( SSc ) , but the precise mechanisms are poorly understood .
	manualset3
192237	5	415655	7	NULL	NULL	0	NULL	systemic sclerosis ( SSc )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Transforming growth factor - ( TGF - ) signaling is implicated in the pathogenesis of fibrosis in scleroderma or systemic sclerosis ( SSc ) , but the precise mechanisms are poorly understood .
	manualset3
192238	6	415655	7	NULL	NULL	0	NULL	mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transforming growth factor - ( TGF - ) signaling is implicated in the pathogenesis of fibrosis in scleroderma or systemic sclerosis ( SSc ) , but the precise mechanisms are poorly understood .
	manualset3
192239	1	415656	7	NULL	NULL	0	NULL	in vitro testing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After in vitro testing of linearity , in vivo infusion studies were performed .
	manualset3
192240	2	415656	7	NULL	NULL	0	NULL	 linearity	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	After in vitro testing of linearity , in vivo infusion studies were performed .
	manualset3
192241	3	415656	7	NULL	NULL	0	NULL	 in vivo infusion studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After in vitro testing of linearity , in vivo infusion studies were performed .
	manualset3
192242	1	415657	7	NULL	NULL	0	NULL	Transforming growth factor alpha levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transforming growth factor alpha and epidermal growth factor levels in normal human gastrointestinal mucosa .
	manualset3
192243	2	415657	7	NULL	NULL	0	NULL	epidermal growth factor levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transforming growth factor alpha and epidermal growth factor levels in normal human gastrointestinal mucosa .
	manualset3
192244	3	415657	7	NULL	NULL	0	NULL	normal human gastrointestinal mucosa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Transforming growth factor alpha and epidermal growth factor levels in normal human gastrointestinal mucosa .
	manualset3
192245	1	415658	7	NULL	NULL	NULL	NULL	Transgender	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Transgender were significantly more likely than gay men , lesbians , and bisexuals to experience discrimination or victimization events .
	manualset3
192246	2	415658	7	NULL	NULL	0	NULL	gay men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Transgender were significantly more likely than gay men , lesbians , and bisexuals to experience discrimination or victimization events .
	manualset3
192247	3	415658	7	NULL	NULL	0	NULL	 lesbians 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Transgender were significantly more likely than gay men , lesbians , and bisexuals to experience discrimination or victimization events .
	manualset3
192248	4	415658	7	NULL	NULL	0	NULL	bisexuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Transgender were significantly more likely than gay men , lesbians , and bisexuals to experience discrimination or victimization events .
	manualset3
192249	5	415658	7	NULL	NULL	0	NULL	discrimination events	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Transgender were significantly more likely than gay men , lesbians , and bisexuals to experience discrimination or victimization events .
	manualset3
192250	6	415658	7	NULL	NULL	0	NULL	victimization events	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Transgender were significantly more likely than gay men , lesbians , and bisexuals to experience discrimination or victimization events .
	manualset3
192251	1	415659	7	NULL	NULL	0	NULL	Transgenic Keratin14-rtTA-PTR mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Transgenic Keratin14-rtTA-PTR mice specifically express Keratin14 ( K14 ) in the tongue epithelia , as well as co-express EGFP and the dominant negative Tgfbr2 genes upon treatment with Doxycycline ( Dox ) .
	manualset3
192252	2	415659	7	NULL	NULL	0	NULL	Keratin14 ( K14 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Transgenic Keratin14-rtTA-PTR mice specifically express Keratin14 ( K14 ) in the tongue epithelia , as well as co-express EGFP and the dominant negative Tgfbr2 genes upon treatment with Doxycycline ( Dox ) .
	manualset3
192253	3	415659	7	NULL	NULL	0	NULL	tongue epithelia	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Transgenic Keratin14-rtTA-PTR mice specifically express Keratin14 ( K14 ) in the tongue epithelia , as well as co-express EGFP and the dominant negative Tgfbr2 genes upon treatment with Doxycycline ( Dox ) .
	manualset3
192254	4	415659	7	NULL	NULL	0	NULL	EGFP genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Transgenic Keratin14-rtTA-PTR mice specifically express Keratin14 ( K14 ) in the tongue epithelia , as well as co-express EGFP and the dominant negative Tgfbr2 genes upon treatment with Doxycycline ( Dox ) .
	manualset3
192255	5	415659	7	NULL	NULL	0	NULL	dominant negative Tgfbr2 genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Transgenic Keratin14-rtTA-PTR mice specifically express Keratin14 ( K14 ) in the tongue epithelia , as well as co-express EGFP and the dominant negative Tgfbr2 genes upon treatment with Doxycycline ( Dox ) .
	manualset3
192256	6	415659	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Transgenic Keratin14-rtTA-PTR mice specifically express Keratin14 ( K14 ) in the tongue epithelia , as well as co-express EGFP and the dominant negative Tgfbr2 genes upon treatment with Doxycycline ( Dox ) .
	manualset3
192257	7	415659	7	NULL	NULL	0	NULL	Doxycycline ( Dox )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Transgenic Keratin14-rtTA-PTR mice specifically express Keratin14 ( K14 ) in the tongue epithelia , as well as co-express EGFP and the dominant negative Tgfbr2 genes upon treatment with Doxycycline ( Dox ) .
	manualset3
192258	1	415660	7	NULL	NULL	0	NULL	Transgenic mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Transgenic mice expressing this mutant form of apolipoprotein ( a ) as well as mice expressing wild-type apolipoprotein ( a ) have been created in an inbred mouse strain .
	manualset3
192259	2	415660	7	NULL	NULL	0	NULL	mutant form	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Transgenic mice expressing this mutant form of apolipoprotein ( a ) as well as mice expressing wild-type apolipoprotein ( a ) have been created in an inbred mouse strain .
	manualset3
192260	3	415660	7	NULL	NULL	0	NULL	apolipoprotein ( a ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Transgenic mice expressing this mutant form of apolipoprotein ( a ) as well as mice expressing wild-type apolipoprotein ( a ) have been created in an inbred mouse strain .
	manualset3
192261	4	415660	7	NULL	NULL	0	NULL	 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Transgenic mice expressing this mutant form of apolipoprotein ( a ) as well as mice expressing wild-type apolipoprotein ( a ) have been created in an inbred mouse strain .
	manualset3
192262	5	415660	7	NULL	NULL	0	NULL	wild-type apolipoprotein ( a )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Transgenic mice expressing this mutant form of apolipoprotein ( a ) as well as mice expressing wild-type apolipoprotein ( a ) have been created in an inbred mouse strain .
	manualset3
192263	6	415660	7	NULL	NULL	0	NULL	inbred mouse strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Transgenic mice expressing this mutant form of apolipoprotein ( a ) as well as mice expressing wild-type apolipoprotein ( a ) have been created in an inbred mouse strain .
	manualset3
192264	1	415661	7	NULL	NULL	0	NULL	Transgenic neuronal nitric oxide synthase expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transgenic neuronal nitric oxide synthase expression induces axotomy-like changes in adult motoneurons .
	manualset3
192265	2	415661	7	NULL	NULL	NULL	NULL	axotomy-like changes	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Transgenic neuronal nitric oxide synthase expression induces axotomy-like changes in adult motoneurons .
	manualset3
192266	3	415661	7	NULL	NULL	0	NULL	adult motoneurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Transgenic neuronal nitric oxide synthase expression induces axotomy-like changes in adult motoneurons .
	manualset3
192267	1	415662	7	NULL	NULL	0	NULL	Transgressive segregation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transgressive segregation created novel genotypes that had either higher fitness or lower fitness in certain environments than either parent .
	manualset3
192268	2	415662	7	NULL	NULL	0	NULL	novel genotypes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Transgressive segregation created novel genotypes that had either higher fitness or lower fitness in certain environments than either parent .
	manualset3
192269	3	415662	7	NULL	NULL	0	NULL	higher fitness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Transgressive segregation created novel genotypes that had either higher fitness or lower fitness in certain environments than either parent .
	manualset3
192270	4	415662	7	NULL	NULL	0	NULL	lower fitness 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Transgressive segregation created novel genotypes that had either higher fitness or lower fitness in certain environments than either parent .
	manualset3
192271	5	415662	7	NULL	NULL	0	NULL	environments	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Transgressive segregation created novel genotypes that had either higher fitness or lower fitness in certain environments than either parent .
	manualset3
192272	6	415662	7	NULL	NULL	0	NULL	parent	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Transgressive segregation created novel genotypes that had either higher fitness or lower fitness in certain environments than either parent .
	manualset3
192273	1	415663	7	NULL	NULL	0	NULL	Transient changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transient changes in neuronal cell membrane permeability after blast exposure .
	manualset3
192274	2	415663	7	NULL	NULL	0	NULL	neuronal cell membrane permeability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transient changes in neuronal cell membrane permeability after blast exposure .
	manualset3
192275	3	415663	7	NULL	NULL	0	NULL	 blast exposure	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Transient changes in neuronal cell membrane permeability after blast exposure .
	manualset3
192276	1	415664	7	NULL	NULL	0	NULL	Transient confinement	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transient confinement of a glycosylphosphatidylinositol-anchored protein in the plasma membrane .
	manualset3
192277	2	415664	7	NULL	NULL	0	NULL	glycosylphosphatidylinositol-anchored protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Transient confinement of a glycosylphosphatidylinositol-anchored protein in the plasma membrane .
	manualset3
192278	3	415664	7	NULL	NULL	0	NULL	plasma membrane 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Transient confinement of a glycosylphosphatidylinositol-anchored protein in the plasma membrane .
	manualset3
192279	1	415665	7	NULL	NULL	0	NULL	Concordant congenital alopecia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Concordant congenital alopecia , achromotrichia and transverse palmar line in dizygotic triplets ( two monozygotic males and one female ) ) .
	manualset3
192280	2	415665	7	NULL	NULL	0	NULL	achromotrichia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Concordant congenital alopecia , achromotrichia and transverse palmar line in dizygotic triplets ( two monozygotic males and one female ) ) .
	manualset3
192281	3	415665	7	NULL	NULL	0	NULL	 transverse palmar line	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Concordant congenital alopecia , achromotrichia and transverse palmar line in dizygotic triplets ( two monozygotic males and one female ) ) .
	manualset3
192282	4	415665	7	NULL	NULL	0	NULL	dizygotic triplets	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Concordant congenital alopecia , achromotrichia and transverse palmar line in dizygotic triplets ( two monozygotic males and one female ) ) .
	manualset3
192283	5	415665	7	NULL	NULL	0	NULL	two monozygotic males	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Concordant congenital alopecia , achromotrichia and transverse palmar line in dizygotic triplets ( two monozygotic males and one female ) ) .
	manualset3
192284	6	415665	7	NULL	NULL	0	NULL	one female	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Concordant congenital alopecia , achromotrichia and transverse palmar line in dizygotic triplets ( two monozygotic males and one female ) ) .
	manualset3
192285	1	415666	7	NULL	NULL	0	NULL	induction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After induction of acrosome reaction , a Hsp70 redistribution in boar spermatozoa and an increased percentage of stallion spermatozoa showing the post-acrosomal signal were observed although no changes were recorded by Western blot ; in dog spermatozoa , no changes in Hsp70 were found by Western blot and immunofluorescence after capacitation and acrosome reaction .
	manualset3
192286	2	415666	7	NULL	NULL	0	NULL	acrosome reaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After induction of acrosome reaction , a Hsp70 redistribution in boar spermatozoa and an increased percentage of stallion spermatozoa showing the post-acrosomal signal were observed although no changes were recorded by Western blot ; in dog spermatozoa , no changes in Hsp70 were found by Western blot and immunofluorescence after capacitation and acrosome reaction .
	manualset3
192287	3	415666	7	NULL	NULL	0	NULL	Hsp70 redistribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After induction of acrosome reaction , a Hsp70 redistribution in boar spermatozoa and an increased percentage of stallion spermatozoa showing the post-acrosomal signal were observed although no changes were recorded by Western blot ; in dog spermatozoa , no changes in Hsp70 were found by Western blot and immunofluorescence after capacitation and acrosome reaction .
	manualset3
192288	4	415666	7	NULL	NULL	0	NULL	boar spermatozoa	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	After induction of acrosome reaction , a Hsp70 redistribution in boar spermatozoa and an increased percentage of stallion spermatozoa showing the post-acrosomal signal were observed although no changes were recorded by Western blot ; in dog spermatozoa , no changes in Hsp70 were found by Western blot and immunofluorescence after capacitation and acrosome reaction .
	manualset3
192289	5	415666	7	NULL	NULL	0	NULL	 increased percentage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After induction of acrosome reaction , a Hsp70 redistribution in boar spermatozoa and an increased percentage of stallion spermatozoa showing the post-acrosomal signal were observed although no changes were recorded by Western blot ; in dog spermatozoa , no changes in Hsp70 were found by Western blot and immunofluorescence after capacitation and acrosome reaction .
	manualset3
192290	6	415666	7	NULL	NULL	0	NULL	stallion spermatozoa	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	After induction of acrosome reaction , a Hsp70 redistribution in boar spermatozoa and an increased percentage of stallion spermatozoa showing the post-acrosomal signal were observed although no changes were recorded by Western blot ; in dog spermatozoa , no changes in Hsp70 were found by Western blot and immunofluorescence after capacitation and acrosome reaction .
	manualset3
192291	7	415666	7	NULL	NULL	0	NULL	post-acrosomal signal	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After induction of acrosome reaction , a Hsp70 redistribution in boar spermatozoa and an increased percentage of stallion spermatozoa showing the post-acrosomal signal were observed although no changes were recorded by Western blot ; in dog spermatozoa , no changes in Hsp70 were found by Western blot and immunofluorescence after capacitation and acrosome reaction .
	manualset3
192292	8	415666	7	NULL	NULL	0	NULL	no changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After induction of acrosome reaction , a Hsp70 redistribution in boar spermatozoa and an increased percentage of stallion spermatozoa showing the post-acrosomal signal were observed although no changes were recorded by Western blot ; in dog spermatozoa , no changes in Hsp70 were found by Western blot and immunofluorescence after capacitation and acrosome reaction .
	manualset3
192293	9	415666	7	NULL	NULL	0	NULL	Western blot	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After induction of acrosome reaction , a Hsp70 redistribution in boar spermatozoa and an increased percentage of stallion spermatozoa showing the post-acrosomal signal were observed although no changes were recorded by Western blot ; in dog spermatozoa , no changes in Hsp70 were found by Western blot and immunofluorescence after capacitation and acrosome reaction .
	manualset3
192294	10	415666	7	NULL	NULL	0	NULL	dog spermatozoa	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	After induction of acrosome reaction , a Hsp70 redistribution in boar spermatozoa and an increased percentage of stallion spermatozoa showing the post-acrosomal signal were observed although no changes were recorded by Western blot ; in dog spermatozoa , no changes in Hsp70 were found by Western blot and immunofluorescence after capacitation and acrosome reaction .
	manualset3
192295	11	415666	7	NULL	NULL	0	NULL	no changes 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After induction of acrosome reaction , a Hsp70 redistribution in boar spermatozoa and an increased percentage of stallion spermatozoa showing the post-acrosomal signal were observed although no changes were recorded by Western blot ; in dog spermatozoa , no changes in Hsp70 were found by Western blot and immunofluorescence after capacitation and acrosome reaction .
	manualset3
192296	12	415666	7	NULL	NULL	0	NULL	Hsp70	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	After induction of acrosome reaction , a Hsp70 redistribution in boar spermatozoa and an increased percentage of stallion spermatozoa showing the post-acrosomal signal were observed although no changes were recorded by Western blot ; in dog spermatozoa , no changes in Hsp70 were found by Western blot and immunofluorescence after capacitation and acrosome reaction .
	manualset3
192297	13	415666	7	NULL	NULL	0	NULL	Western blot	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After induction of acrosome reaction , a Hsp70 redistribution in boar spermatozoa and an increased percentage of stallion spermatozoa showing the post-acrosomal signal were observed although no changes were recorded by Western blot ; in dog spermatozoa , no changes in Hsp70 were found by Western blot and immunofluorescence after capacitation and acrosome reaction .
	manualset3
192298	14	415666	7	NULL	NULL	0	NULL	immunofluorescence 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After induction of acrosome reaction , a Hsp70 redistribution in boar spermatozoa and an increased percentage of stallion spermatozoa showing the post-acrosomal signal were observed although no changes were recorded by Western blot ; in dog spermatozoa , no changes in Hsp70 were found by Western blot and immunofluorescence after capacitation and acrosome reaction .
	manualset3
192299	15	415666	7	NULL	NULL	NULL	NULL	capacitation 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After induction of acrosome reaction , a Hsp70 redistribution in boar spermatozoa and an increased percentage of stallion spermatozoa showing the post-acrosomal signal were observed although no changes were recorded by Western blot ; in dog spermatozoa , no changes in Hsp70 were found by Western blot and immunofluorescence after capacitation and acrosome reaction .
	manualset3
192300	16	415666	7	NULL	NULL	0	NULL	acrosome reaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After induction of acrosome reaction , a Hsp70 redistribution in boar spermatozoa and an increased percentage of stallion spermatozoa showing the post-acrosomal signal were observed although no changes were recorded by Western blot ; in dog spermatozoa , no changes in Hsp70 were found by Western blot and immunofluorescence after capacitation and acrosome reaction .
	manualset3
192301	1	415667	7	NULL	NULL	0	NULL	Transient exacerbation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Transient exacerbation of skin condition with a peak between the 2nd and 6th day of treatment could be observed in three patients .
	manualset3
192302	2	415667	7	NULL	NULL	0	NULL	skin condition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Transient exacerbation of skin condition with a peak between the 2nd and 6th day of treatment could be observed in three patients .
	manualset3
192303	3	415667	7	NULL	NULL	0	NULL	peak	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transient exacerbation of skin condition with a peak between the 2nd and 6th day of treatment could be observed in three patients .
	manualset3
192304	4	415667	7	NULL	NULL	0	NULL	2nd day	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Transient exacerbation of skin condition with a peak between the 2nd and 6th day of treatment could be observed in three patients .
	manualset3
192305	5	415667	7	NULL	NULL	0	NULL	6th day	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Transient exacerbation of skin condition with a peak between the 2nd and 6th day of treatment could be observed in three patients .
	manualset3
192306	6	415667	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Transient exacerbation of skin condition with a peak between the 2nd and 6th day of treatment could be observed in three patients .
	manualset3
192307	7	415667	7	NULL	NULL	0	NULL	three patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Transient exacerbation of skin condition with a peak between the 2nd and 6th day of treatment could be observed in three patients .
	manualset3
192308	1	415668	7	NULL	NULL	0	NULL	Transient expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transient expression of alpha4 integrins or L-selectin also increased several fold migration both in vitro and in vivo .
	manualset3
192309	2	415668	7	NULL	NULL	0	NULL	alpha4 integrins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Transient expression of alpha4 integrins or L-selectin also increased several fold migration both in vitro and in vivo .
	manualset3
192310	3	415668	7	NULL	NULL	0	NULL	L-selectin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Transient expression of alpha4 integrins or L-selectin also increased several fold migration both in vitro and in vivo .
	manualset3
192311	4	415668	7	NULL	NULL	0	NULL	several fold migration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transient expression of alpha4 integrins or L-selectin also increased several fold migration both in vitro and in vivo .
	manualset3
192312	1	415669	7	NULL	NULL	0	NULL	Transient expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transient expression of mouse PPT in COS-1 cells yielded a 38/36-kD differentially glycosylated polypeptide that was also secreted into culture media .
	manualset3
192313	2	415669	7	NULL	NULL	0	NULL	mouse PPT	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Transient expression of mouse PPT in COS-1 cells yielded a 38/36-kD differentially glycosylated polypeptide that was also secreted into culture media .
	manualset3
192314	3	415669	7	NULL	NULL	0	NULL	COS-1 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Transient expression of mouse PPT in COS-1 cells yielded a 38/36-kD differentially glycosylated polypeptide that was also secreted into culture media .
	manualset3
192315	4	415669	7	NULL	NULL	0	NULL	38/36-kD	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transient expression of mouse PPT in COS-1 cells yielded a 38/36-kD differentially glycosylated polypeptide that was also secreted into culture media .
	manualset3
192316	5	415669	7	NULL	NULL	0	NULL	glycosylated polypeptide	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Transient expression of mouse PPT in COS-1 cells yielded a 38/36-kD differentially glycosylated polypeptide that was also secreted into culture media .
	manualset3
192317	6	415669	7	NULL	NULL	0	NULL	culture media	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Transient expression of mouse PPT in COS-1 cells yielded a 38/36-kD differentially glycosylated polypeptide that was also secreted into culture media .
	manualset3
192318	1	415670	7	NULL	NULL	0	NULL	Transient receptor potential ( TRP ) channels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Transient receptor potential ( TRP ) channels of multiple subclasses are expressed in the heart , although their functions are only now beginning to emerge , especially for the TRPC subclass that appears to regulate the cardiac hypertrophic response .
	manualset3
192319	2	415670	7	NULL	NULL	0	NULL	multiple subclasses	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Transient receptor potential ( TRP ) channels of multiple subclasses are expressed in the heart , although their functions are only now beginning to emerge , especially for the TRPC subclass that appears to regulate the cardiac hypertrophic response .
	manualset3
192320	3	415670	7	NULL	NULL	0	NULL	heart	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Transient receptor potential ( TRP ) channels of multiple subclasses are expressed in the heart , although their functions are only now beginning to emerge , especially for the TRPC subclass that appears to regulate the cardiac hypertrophic response .
	manualset3
192321	4	415670	7	NULL	NULL	0	NULL	functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transient receptor potential ( TRP ) channels of multiple subclasses are expressed in the heart , although their functions are only now beginning to emerge , especially for the TRPC subclass that appears to regulate the cardiac hypertrophic response .
	manualset3
192322	5	415670	7	NULL	NULL	0	NULL	TRPC subclass 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Transient receptor potential ( TRP ) channels of multiple subclasses are expressed in the heart , although their functions are only now beginning to emerge , especially for the TRPC subclass that appears to regulate the cardiac hypertrophic response .
	manualset3
192323	6	415670	7	NULL	NULL	0	NULL	cardiac hypertrophic response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Transient receptor potential ( TRP ) channels of multiple subclasses are expressed in the heart , although their functions are only now beginning to emerge , especially for the TRPC subclass that appears to regulate the cardiac hypertrophic response .
	manualset3
192324	1	415671	7	NULL	NULL	0	NULL	Translation initiation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Translation initiation of Hsp83 at all temperatures appears to proceed via scanning of the 5 ' UTR , since a hairpin structure abolishes expression of a fused reporter gene .
	manualset3
192325	2	415671	7	NULL	NULL	0	NULL	Hsp83	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Translation initiation of Hsp83 at all temperatures appears to proceed via scanning of the 5 ' UTR , since a hairpin structure abolishes expression of a fused reporter gene .
	manualset3
192326	3	415671	7	NULL	NULL	0	NULL	temperatures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Translation initiation of Hsp83 at all temperatures appears to proceed via scanning of the 5 ' UTR , since a hairpin structure abolishes expression of a fused reporter gene .
	manualset3
192327	4	415671	7	NULL	NULL	0	NULL	scanning	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Translation initiation of Hsp83 at all temperatures appears to proceed via scanning of the 5 ' UTR , since a hairpin structure abolishes expression of a fused reporter gene .
	manualset3
192328	5	415671	7	NULL	NULL	0	NULL	5 ' UTR 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Translation initiation of Hsp83 at all temperatures appears to proceed via scanning of the 5 ' UTR , since a hairpin structure abolishes expression of a fused reporter gene .
	manualset3
192329	6	415671	7	NULL	NULL	0	NULL	hairpin structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Translation initiation of Hsp83 at all temperatures appears to proceed via scanning of the 5 ' UTR , since a hairpin structure abolishes expression of a fused reporter gene .
	manualset3
192330	7	415671	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Translation initiation of Hsp83 at all temperatures appears to proceed via scanning of the 5 ' UTR , since a hairpin structure abolishes expression of a fused reporter gene .
	manualset3
192331	8	415671	7	NULL	NULL	0	NULL	fused reporter gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Translation initiation of Hsp83 at all temperatures appears to proceed via scanning of the 5 ' UTR , since a hairpin structure abolishes expression of a fused reporter gene .
	manualset3
192442	1	415672	7	NULL	NULL	0	NULL	Translation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Translation of mRNA for some expressed genes , including HSP70 and HSP40 , was corroborated by Western blotting .
	manualset3
192443	2	415672	7	NULL	NULL	0	NULL	mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Translation of mRNA for some expressed genes , including HSP70 and HSP40 , was corroborated by Western blotting .
	manualset3
192444	3	415672	7	NULL	NULL	0	NULL	expressed genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Translation of mRNA for some expressed genes , including HSP70 and HSP40 , was corroborated by Western blotting .
	manualset3
192445	4	415672	7	NULL	NULL	0	NULL	HSP70	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Translation of mRNA for some expressed genes , including HSP70 and HSP40 , was corroborated by Western blotting .
	manualset3
192446	5	415672	7	NULL	NULL	0	NULL	HSP40	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Translation of mRNA for some expressed genes , including HSP70 and HSP40 , was corroborated by Western blotting .
	manualset3
192447	6	415672	7	NULL	NULL	0	NULL	Western blotting	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Translation of mRNA for some expressed genes , including HSP70 and HSP40 , was corroborated by Western blotting .
	manualset3
192448	1	415673	7	NULL	NULL	0	NULL	infancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After infancy , all of the growth modalities were positively associated with systolic BP ( weight , 1.91 ; weight-for-height , 1.56 ; height , 1.20 mm Hg SD ( -1 ) ; all P & lt ; 0.001 ) .
	manualset3
192449	2	415673	7	NULL	NULL	0	NULL	growth modalities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After infancy , all of the growth modalities were positively associated with systolic BP ( weight , 1.91 ; weight-for-height , 1.56 ; height , 1.20 mm Hg SD ( -1 ) ; all P & lt ; 0.001 ) .
	manualset3
192450	3	415673	7	NULL	NULL	0	NULL	systolic BP	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After infancy , all of the growth modalities were positively associated with systolic BP ( weight , 1.91 ; weight-for-height , 1.56 ; height , 1.20 mm Hg SD ( -1 ) ; all P & lt ; 0.001 ) .
	manualset3
192451	4	415673	7	NULL	NULL	0	NULL	weight , 1.91	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After infancy , all of the growth modalities were positively associated with systolic BP ( weight , 1.91 ; weight-for-height , 1.56 ; height , 1.20 mm Hg SD ( -1 ) ; all P & lt ; 0.001 ) .
	manualset3
192452	5	415673	7	NULL	NULL	0	NULL	weight-for-height	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After infancy , all of the growth modalities were positively associated with systolic BP ( weight , 1.91 ; weight-for-height , 1.56 ; height , 1.20 mm Hg SD ( -1 ) ; all P & lt ; 0.001 ) .
	manualset3
192453	6	415673	7	NULL	NULL	NULL	NULL	1.56 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After infancy , all of the growth modalities were positively associated with systolic BP ( weight , 1.91 ; weight-for-height , 1.56 ; height , 1.20 mm Hg SD ( -1 ) ; all P & lt ; 0.001 ) .
	manualset3
192454	7	415673	7	NULL	NULL	NULL	NULL	height 1.20 mm Hg SD ( -1 )	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After infancy , all of the growth modalities were positively associated with systolic BP ( weight , 1.91 ; weight-for-height , 1.56 ; height , 1.20 mm Hg SD ( -1 ) ; all P & lt ; 0.001 ) .
	manualset3
192455	8	415673	7	NULL	NULL	0	NULL	P & lt ; 0.001	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After infancy , all of the growth modalities were positively associated with systolic BP ( weight , 1.91 ; weight-for-height , 1.56 ; height , 1.20 mm Hg SD ( -1 ) ; all P & lt ; 0.001 ) .
	manualset3
192456	1	415674	7	NULL	NULL	NULL	NULL	Transmalleolar approach	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Transmalleolar approach to a tubercular lytic lesion of the talar body : a case report .
	manualset3
192457	2	415674	7	NULL	NULL	0	NULL	tubercular lytic lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Transmalleolar approach to a tubercular lytic lesion of the talar body : a case report .
	manualset3
192458	3	415674	7	NULL	NULL	0	NULL	talar body	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Transmalleolar approach to a tubercular lytic lesion of the talar body : a case report .
	manualset3
192459	4	415674	7	NULL	NULL	0	NULL	case report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Transmalleolar approach to a tubercular lytic lesion of the talar body : a case report .
	manualset3
192460	1	415675	7	NULL	NULL	0	NULL	Transmembrane protein 147 ( TMEM147 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Transmembrane protein 147 ( TMEM147 ) is a novel component of the Nicalin-NOMO protein complex .
	manualset3
192461	2	415675	7	NULL	NULL	0	NULL	novel component	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Transmembrane protein 147 ( TMEM147 ) is a novel component of the Nicalin-NOMO protein complex .
	manualset3
192462	3	415675	7	NULL	NULL	NULL	NULL	Nicalin-NOMO protein complex	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Transmembrane protein 147 ( TMEM147 ) is a novel component of the Nicalin-NOMO protein complex .
	manualset3
192463	1	415676	7	NULL	NULL	0	NULL	Transmission electron microscopy studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transmission electron microscopy studies show that the crystal grain size of MgF ( 2 ) films is not strongly affected by oxygen or argon-ion bombardment .
	manualset3
192464	2	415676	7	NULL	NULL	0	NULL	crystal grain size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transmission electron microscopy studies show that the crystal grain size of MgF ( 2 ) films is not strongly affected by oxygen or argon-ion bombardment .
	manualset3
192465	3	415676	7	NULL	NULL	0	NULL	MgF ( 2 ) films 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Transmission electron microscopy studies show that the crystal grain size of MgF ( 2 ) films is not strongly affected by oxygen or argon-ion bombardment .
	manualset3
192466	4	415676	7	NULL	NULL	0	NULL	oxygen	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Transmission electron microscopy studies show that the crystal grain size of MgF ( 2 ) films is not strongly affected by oxygen or argon-ion bombardment .
	manualset3
192467	5	415676	7	NULL	NULL	0	NULL	argon-ion bombardment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Transmission electron microscopy studies show that the crystal grain size of MgF ( 2 ) films is not strongly affected by oxygen or argon-ion bombardment .
	manualset3
192468	1	415677	7	NULL	NULL	0	NULL	Transmitral Doppler flow	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Transmitral Doppler flow should be evaluated in combination with newer , less load dependent Doppler techniques .
	manualset3
192469	2	415677	7	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Transmitral Doppler flow should be evaluated in combination with newer , less load dependent Doppler techniques .
	manualset3
192470	3	415677	7	NULL	NULL	0	NULL	less load dependent Doppler techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transmitral Doppler flow should be evaluated in combination with newer , less load dependent Doppler techniques .
	manualset3
192471	1	415678	7	NULL	NULL	0	NULL	Transplacental CO uptake ( VCO ) 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transplacental CO uptake ( VCO ) was determined as the product of fetal blood CO content and fetal CO space ( 11.8 % of fetal weight ) .
	manualset3
192472	2	415678	7	NULL	NULL	NULL	NULL	product 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Transplacental CO uptake ( VCO ) was determined as the product of fetal blood CO content and fetal CO space ( 11.8 % of fetal weight ) .
	manualset3
192473	3	415678	7	NULL	NULL	0	NULL	 fetal blood CO content 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transplacental CO uptake ( VCO ) was determined as the product of fetal blood CO content and fetal CO space ( 11.8 % of fetal weight ) .
	manualset3
192474	4	415678	7	NULL	NULL	0	NULL	fetal CO space	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transplacental CO uptake ( VCO ) was determined as the product of fetal blood CO content and fetal CO space ( 11.8 % of fetal weight ) .
	manualset3
192475	5	415678	7	NULL	NULL	NULL	NULL	11.8 % 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Transplacental CO uptake ( VCO ) was determined as the product of fetal blood CO content and fetal CO space ( 11.8 % of fetal weight ) .
	manualset3
192476	6	415678	7	NULL	NULL	0	NULL	fetal weight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transplacental CO uptake ( VCO ) was determined as the product of fetal blood CO content and fetal CO space ( 11.8 % of fetal weight ) .
	manualset3
192477	1	415679	7	NULL	NULL	0	NULL	Transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Transplantation in the management of metastatic endocrine tumors .
	manualset3
192478	2	415679	7	NULL	NULL	0	NULL	management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Transplantation in the management of metastatic endocrine tumors .
	manualset3
192479	3	415679	7	NULL	NULL	0	NULL	metastatic endocrine tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Transplantation in the management of metastatic endocrine tumors .
	manualset3
192480	1	415680	7	NULL	NULL	0	NULL	Transplantation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Transplantation of bone marrow cells partially corrects the metabolic phenotype in a mouse model for Wilson 's disease .
	manualset3
192481	2	415680	7	NULL	NULL	0	NULL	bone marrow cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Transplantation of bone marrow cells partially corrects the metabolic phenotype in a mouse model for Wilson 's disease .
	manualset3
192482	3	415680	7	NULL	NULL	0	NULL	metabolic phenotype	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transplantation of bone marrow cells partially corrects the metabolic phenotype in a mouse model for Wilson 's disease .
	manualset3
192483	4	415680	7	NULL	NULL	0	NULL	mouse model	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Transplantation of bone marrow cells partially corrects the metabolic phenotype in a mouse model for Wilson 's disease .
	manualset3
192484	5	415680	7	NULL	NULL	0	NULL	Wilson 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Transplantation of bone marrow cells partially corrects the metabolic phenotype in a mouse model for Wilson 's disease .
	manualset3
192485	1	415681	7	NULL	NULL	0	NULL	informed consent salbutamol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	After informed consent salbutamol was well tolerated but the patient had asthma in 5 min of manipulation of the lupine seeds .
	manualset3
192486	2	415681	7	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	After informed consent salbutamol was well tolerated but the patient had asthma in 5 min of manipulation of the lupine seeds .
	manualset3
192487	3	415681	7	NULL	NULL	0	NULL	asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	After informed consent salbutamol was well tolerated but the patient had asthma in 5 min of manipulation of the lupine seeds .
	manualset3
192488	4	415681	7	NULL	NULL	0	NULL	 5 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After informed consent salbutamol was well tolerated but the patient had asthma in 5 min of manipulation of the lupine seeds .
	manualset3
192489	5	415681	7	NULL	NULL	0	NULL	manipulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After informed consent salbutamol was well tolerated but the patient had asthma in 5 min of manipulation of the lupine seeds .
	manualset3
192490	6	415681	7	NULL	NULL	NULL	NULL	lupine seeds	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After informed consent salbutamol was well tolerated but the patient had asthma in 5 min of manipulation of the lupine seeds .
	manualset3
192491	1	415682	7	NULL	NULL	0	NULL	transport 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transport of - casozepine across Caco-2 monolayer increased significantly , in the presence of bile extract , and of fragment f91-97 , in the presence of bile salts .
	manualset3
192492	2	415682	7	NULL	NULL	0	NULL	 casozepine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Transport of - casozepine across Caco-2 monolayer increased significantly , in the presence of bile extract , and of fragment f91-97 , in the presence of bile salts .
	manualset3
192493	3	415682	7	NULL	NULL	0	NULL	Caco-2 monolayer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Transport of - casozepine across Caco-2 monolayer increased significantly , in the presence of bile extract , and of fragment f91-97 , in the presence of bile salts .
	manualset3
192494	4	415682	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Transport of - casozepine across Caco-2 monolayer increased significantly , in the presence of bile extract , and of fragment f91-97 , in the presence of bile salts .
	manualset3
192495	5	415682	7	NULL	NULL	0	NULL	bile extract	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Transport of - casozepine across Caco-2 monolayer increased significantly , in the presence of bile extract , and of fragment f91-97 , in the presence of bile salts .
	manualset3
192496	6	415682	7	NULL	NULL	0	NULL	fragment	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Transport of - casozepine across Caco-2 monolayer increased significantly , in the presence of bile extract , and of fragment f91-97 , in the presence of bile salts .
	manualset3
192497	7	415682	7	NULL	NULL	0	NULL	 f91-97	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Transport of - casozepine across Caco-2 monolayer increased significantly , in the presence of bile extract , and of fragment f91-97 , in the presence of bile salts .
	manualset3
192498	8	415682	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Transport of - casozepine across Caco-2 monolayer increased significantly , in the presence of bile extract , and of fragment f91-97 , in the presence of bile salts .
	manualset3
192499	9	415682	7	NULL	NULL	0	NULL	bile salts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Transport of - casozepine across Caco-2 monolayer increased significantly , in the presence of bile extract , and of fragment f91-97 , in the presence of bile salts .
	manualset3
192500	1	415683	7	NULL	NULL	0	NULL	Transport	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transport of solute and water across the peritoneum is measured via a plastic chamber affixed to the abdominal wall of anesthetized Sprague-Dawley rats .
	manualset3
192501	2	415683	7	NULL	NULL	NULL	NULL	solute	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Transport of solute and water across the peritoneum is measured via a plastic chamber affixed to the abdominal wall of anesthetized Sprague-Dawley rats .
	manualset3
192502	3	415683	7	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Transport of solute and water across the peritoneum is measured via a plastic chamber affixed to the abdominal wall of anesthetized Sprague-Dawley rats .
	manualset3
192503	4	415683	7	NULL	NULL	0	NULL	peritoneum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Transport of solute and water across the peritoneum is measured via a plastic chamber affixed to the abdominal wall of anesthetized Sprague-Dawley rats .
	manualset3
192504	5	415683	7	NULL	NULL	0	NULL	plastic chamber	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Transport of solute and water across the peritoneum is measured via a plastic chamber affixed to the abdominal wall of anesthetized Sprague-Dawley rats .
	manualset3
192505	6	415683	7	NULL	NULL	0	NULL	abdominal wall 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Transport of solute and water across the peritoneum is measured via a plastic chamber affixed to the abdominal wall of anesthetized Sprague-Dawley rats .
	manualset3
192506	7	415683	7	NULL	NULL	0	NULL	anesthetized Sprague-Dawley rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Transport of solute and water across the peritoneum is measured via a plastic chamber affixed to the abdominal wall of anesthetized Sprague-Dawley rats .
	manualset3
192507	1	415684	7	NULL	NULL	0	NULL	Transposition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transposition of ampicillin Tn1 transposon is repressed under normal conditions and occurs with low frequency ( 10 ( -4 ) per cell ) .
	manualset3
192508	2	415684	7	NULL	NULL	0	NULL	ampicillin Tn1 transposon	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Transposition of ampicillin Tn1 transposon is repressed under normal conditions and occurs with low frequency ( 10 ( -4 ) per cell ) .
	manualset3
192509	3	415684	7	NULL	NULL	0	NULL	normal conditions 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Transposition of ampicillin Tn1 transposon is repressed under normal conditions and occurs with low frequency ( 10 ( -4 ) per cell ) .
	manualset3
192510	4	415684	7	NULL	NULL	0	NULL	 low frequency 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transposition of ampicillin Tn1 transposon is repressed under normal conditions and occurs with low frequency ( 10 ( -4 ) per cell ) .
	manualset3
192511	5	415684	7	NULL	NULL	0	NULL	10 ( -4 ) per cell	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Transposition of ampicillin Tn1 transposon is repressed under normal conditions and occurs with low frequency ( 10 ( -4 ) per cell ) .
	manualset3
192512	1	415685	7	NULL	NULL	0	NULL	Transthoracic echocardiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Transthoracic and transesophageal echocardiography were performed in all subjects to measure the following : left ventricular dimension , interventricular septal thickness and peak velocity at the left ventricular outflow tract by transthoracic echocardiography ; the lengths and the thicknesses of the rough zone of the anterior and posterior mitral leaflets at mid-diastole and the distance between the tip of the posterior papillary muscle and the anterior mitral annulus by transesophageal echocardiography .
	manualset3
192513	2	415685	7	NULL	NULL	0	NULL	transesophageal echocardiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Transthoracic and transesophageal echocardiography were performed in all subjects to measure the following : left ventricular dimension , interventricular septal thickness and peak velocity at the left ventricular outflow tract by transthoracic echocardiography ; the lengths and the thicknesses of the rough zone of the anterior and posterior mitral leaflets at mid-diastole and the distance between the tip of the posterior papillary muscle and the anterior mitral annulus by transesophageal echocardiography .
	manualset3
192514	3	415685	7	NULL	NULL	0	NULL	subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Transthoracic and transesophageal echocardiography were performed in all subjects to measure the following : left ventricular dimension , interventricular septal thickness and peak velocity at the left ventricular outflow tract by transthoracic echocardiography ; the lengths and the thicknesses of the rough zone of the anterior and posterior mitral leaflets at mid-diastole and the distance between the tip of the posterior papillary muscle and the anterior mitral annulus by transesophageal echocardiography .
	manualset3
192515	4	415685	7	NULL	NULL	0	NULL	 following 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transthoracic and transesophageal echocardiography were performed in all subjects to measure the following : left ventricular dimension , interventricular septal thickness and peak velocity at the left ventricular outflow tract by transthoracic echocardiography ; the lengths and the thicknesses of the rough zone of the anterior and posterior mitral leaflets at mid-diastole and the distance between the tip of the posterior papillary muscle and the anterior mitral annulus by transesophageal echocardiography .
	manualset3
192516	5	415685	7	NULL	NULL	0	NULL	 left ventricular dimension	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transthoracic and transesophageal echocardiography were performed in all subjects to measure the following : left ventricular dimension , interventricular septal thickness and peak velocity at the left ventricular outflow tract by transthoracic echocardiography ; the lengths and the thicknesses of the rough zone of the anterior and posterior mitral leaflets at mid-diastole and the distance between the tip of the posterior papillary muscle and the anterior mitral annulus by transesophageal echocardiography .
	manualset3
192517	6	415685	7	NULL	NULL	0	NULL	 interventricular septal thickness	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transthoracic and transesophageal echocardiography were performed in all subjects to measure the following : left ventricular dimension , interventricular septal thickness and peak velocity at the left ventricular outflow tract by transthoracic echocardiography ; the lengths and the thicknesses of the rough zone of the anterior and posterior mitral leaflets at mid-diastole and the distance between the tip of the posterior papillary muscle and the anterior mitral annulus by transesophageal echocardiography .
	manualset3
192518	7	415685	7	NULL	NULL	0	NULL	peak velocity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transthoracic and transesophageal echocardiography were performed in all subjects to measure the following : left ventricular dimension , interventricular septal thickness and peak velocity at the left ventricular outflow tract by transthoracic echocardiography ; the lengths and the thicknesses of the rough zone of the anterior and posterior mitral leaflets at mid-diastole and the distance between the tip of the posterior papillary muscle and the anterior mitral annulus by transesophageal echocardiography .
	manualset3
192519	8	415685	7	NULL	NULL	0	NULL	 left ventricular outflow tract 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Transthoracic and transesophageal echocardiography were performed in all subjects to measure the following : left ventricular dimension , interventricular septal thickness and peak velocity at the left ventricular outflow tract by transthoracic echocardiography ; the lengths and the thicknesses of the rough zone of the anterior and posterior mitral leaflets at mid-diastole and the distance between the tip of the posterior papillary muscle and the anterior mitral annulus by transesophageal echocardiography .
	manualset3
192520	9	415685	7	NULL	NULL	0	NULL	transthoracic echocardiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Transthoracic and transesophageal echocardiography were performed in all subjects to measure the following : left ventricular dimension , interventricular septal thickness and peak velocity at the left ventricular outflow tract by transthoracic echocardiography ; the lengths and the thicknesses of the rough zone of the anterior and posterior mitral leaflets at mid-diastole and the distance between the tip of the posterior papillary muscle and the anterior mitral annulus by transesophageal echocardiography .
	manualset3
192521	10	415685	7	NULL	NULL	0	NULL	lengths	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transthoracic and transesophageal echocardiography were performed in all subjects to measure the following : left ventricular dimension , interventricular septal thickness and peak velocity at the left ventricular outflow tract by transthoracic echocardiography ; the lengths and the thicknesses of the rough zone of the anterior and posterior mitral leaflets at mid-diastole and the distance between the tip of the posterior papillary muscle and the anterior mitral annulus by transesophageal echocardiography .
	manualset3
192522	11	415685	7	NULL	NULL	0	NULL	thicknesses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transthoracic and transesophageal echocardiography were performed in all subjects to measure the following : left ventricular dimension , interventricular septal thickness and peak velocity at the left ventricular outflow tract by transthoracic echocardiography ; the lengths and the thicknesses of the rough zone of the anterior and posterior mitral leaflets at mid-diastole and the distance between the tip of the posterior papillary muscle and the anterior mitral annulus by transesophageal echocardiography .
	manualset3
192523	12	415685	7	NULL	NULL	0	NULL	 rough zone	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Transthoracic and transesophageal echocardiography were performed in all subjects to measure the following : left ventricular dimension , interventricular septal thickness and peak velocity at the left ventricular outflow tract by transthoracic echocardiography ; the lengths and the thicknesses of the rough zone of the anterior and posterior mitral leaflets at mid-diastole and the distance between the tip of the posterior papillary muscle and the anterior mitral annulus by transesophageal echocardiography .
	manualset3
192524	13	415685	7	NULL	NULL	0	NULL	anterior mitral leaflets 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Transthoracic and transesophageal echocardiography were performed in all subjects to measure the following : left ventricular dimension , interventricular septal thickness and peak velocity at the left ventricular outflow tract by transthoracic echocardiography ; the lengths and the thicknesses of the rough zone of the anterior and posterior mitral leaflets at mid-diastole and the distance between the tip of the posterior papillary muscle and the anterior mitral annulus by transesophageal echocardiography .
	manualset3
192525	14	415685	7	NULL	NULL	0	NULL	posterior mitral leaflets	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Transthoracic and transesophageal echocardiography were performed in all subjects to measure the following : left ventricular dimension , interventricular septal thickness and peak velocity at the left ventricular outflow tract by transthoracic echocardiography ; the lengths and the thicknesses of the rough zone of the anterior and posterior mitral leaflets at mid-diastole and the distance between the tip of the posterior papillary muscle and the anterior mitral annulus by transesophageal echocardiography .
	manualset3
192526	15	415685	7	NULL	NULL	0	NULL	 mid-diastole 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Transthoracic and transesophageal echocardiography were performed in all subjects to measure the following : left ventricular dimension , interventricular septal thickness and peak velocity at the left ventricular outflow tract by transthoracic echocardiography ; the lengths and the thicknesses of the rough zone of the anterior and posterior mitral leaflets at mid-diastole and the distance between the tip of the posterior papillary muscle and the anterior mitral annulus by transesophageal echocardiography .
	manualset3
192527	16	415685	7	NULL	NULL	0	NULL	distance	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Transthoracic and transesophageal echocardiography were performed in all subjects to measure the following : left ventricular dimension , interventricular septal thickness and peak velocity at the left ventricular outflow tract by transthoracic echocardiography ; the lengths and the thicknesses of the rough zone of the anterior and posterior mitral leaflets at mid-diastole and the distance between the tip of the posterior papillary muscle and the anterior mitral annulus by transesophageal echocardiography .
	manualset3
192528	17	415685	7	NULL	NULL	0	NULL	 tip	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Transthoracic and transesophageal echocardiography were performed in all subjects to measure the following : left ventricular dimension , interventricular septal thickness and peak velocity at the left ventricular outflow tract by transthoracic echocardiography ; the lengths and the thicknesses of the rough zone of the anterior and posterior mitral leaflets at mid-diastole and the distance between the tip of the posterior papillary muscle and the anterior mitral annulus by transesophageal echocardiography .
	manualset3
192529	18	415685	7	NULL	NULL	0	NULL	posterior papillary muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Transthoracic and transesophageal echocardiography were performed in all subjects to measure the following : left ventricular dimension , interventricular septal thickness and peak velocity at the left ventricular outflow tract by transthoracic echocardiography ; the lengths and the thicknesses of the rough zone of the anterior and posterior mitral leaflets at mid-diastole and the distance between the tip of the posterior papillary muscle and the anterior mitral annulus by transesophageal echocardiography .
	manualset3
192530	19	415685	7	NULL	NULL	0	NULL	anterior mitral annulus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Transthoracic and transesophageal echocardiography were performed in all subjects to measure the following : left ventricular dimension , interventricular septal thickness and peak velocity at the left ventricular outflow tract by transthoracic echocardiography ; the lengths and the thicknesses of the rough zone of the anterior and posterior mitral leaflets at mid-diastole and the distance between the tip of the posterior papillary muscle and the anterior mitral annulus by transesophageal echocardiography .
	manualset3
192531	20	415685	7	NULL	NULL	0	NULL	 transesophageal echocardiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Transthoracic and transesophageal echocardiography were performed in all subjects to measure the following : left ventricular dimension , interventricular septal thickness and peak velocity at the left ventricular outflow tract by transthoracic echocardiography ; the lengths and the thicknesses of the rough zone of the anterior and posterior mitral leaflets at mid-diastole and the distance between the tip of the posterior papillary muscle and the anterior mitral annulus by transesophageal echocardiography .
	manualset3
192532	1	415686	7	NULL	NULL	0	NULL	Transthoracic ultrasonography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Transthoracic ultrasonography to diagnose pneumothorax in trauma .
	manualset3
192533	2	415686	7	NULL	NULL	0	NULL	pneumothorax	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Transthoracic ultrasonography to diagnose pneumothorax in trauma .
	manualset3
192534	3	415686	7	NULL	NULL	0	NULL	 trauma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Transthoracic ultrasonography to diagnose pneumothorax in trauma .
	manualset3
192535	1	415687	7	NULL	NULL	0	NULL	Trapping 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Trapping , stabilization , and characterization of an enolate anion of a 1 , 6-adduct of benzophenone chelated by a sodium alkylamidozincate cation .
	manualset3
192536	2	415687	7	NULL	NULL	0	NULL	stabilization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Trapping , stabilization , and characterization of an enolate anion of a 1 , 6-adduct of benzophenone chelated by a sodium alkylamidozincate cation .
	manualset3
192537	3	415687	7	NULL	NULL	0	NULL	characterization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Trapping , stabilization , and characterization of an enolate anion of a 1 , 6-adduct of benzophenone chelated by a sodium alkylamidozincate cation .
	manualset3
192538	4	415687	7	NULL	NULL	0	NULL	enolate anion	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Trapping , stabilization , and characterization of an enolate anion of a 1 , 6-adduct of benzophenone chelated by a sodium alkylamidozincate cation .
	manualset3
192539	5	415687	7	NULL	NULL	0	NULL	1 , 6-adduct of benzophenone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Trapping , stabilization , and characterization of an enolate anion of a 1 , 6-adduct of benzophenone chelated by a sodium alkylamidozincate cation .
	manualset3
192540	6	415687	7	NULL	NULL	0	NULL	sodium alkylamidozincate cation	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Trapping , stabilization , and characterization of an enolate anion of a 1 , 6-adduct of benzophenone chelated by a sodium alkylamidozincate cation .
	manualset3
192541	1	415688	7	NULL	NULL	0	NULL	Trapping	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Trapping of larvae was observed in mice receiving a sensitization dose of 25 or more eggs .
	manualset3
192542	2	415688	7	NULL	NULL	0	NULL	larvae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Trapping of larvae was observed in mice receiving a sensitization dose of 25 or more eggs .
	manualset3
192543	3	415688	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Trapping of larvae was observed in mice receiving a sensitization dose of 25 or more eggs .
	manualset3
192544	4	415688	7	NULL	NULL	0	NULL	sensitization dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Trapping of larvae was observed in mice receiving a sensitization dose of 25 or more eggs .
	manualset3
192545	5	415688	7	NULL	NULL	NULL	NULL	25	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Trapping of larvae was observed in mice receiving a sensitization dose of 25 or more eggs .
	manualset3
192546	6	415688	7	NULL	NULL	0	NULL	eggs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Trapping of larvae was observed in mice receiving a sensitization dose of 25 or more eggs .
	manualset3
192547	1	415689	7	NULL	NULL	0	NULL	Traumatic coronary artery-cameral fistulas ( TCAF )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Traumatic coronary artery-cameral fistulas ( TCAF ) are uncommon sequelae of trauma that require early surgical intervention to prevent complications .
	manualset3
192548	2	415689	7	NULL	NULL	0	NULL	 uncommon sequelae	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Traumatic coronary artery-cameral fistulas ( TCAF ) are uncommon sequelae of trauma that require early surgical intervention to prevent complications .
	manualset3
192549	3	415689	7	NULL	NULL	0	NULL	 trauma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Traumatic coronary artery-cameral fistulas ( TCAF ) are uncommon sequelae of trauma that require early surgical intervention to prevent complications .
	manualset3
192550	4	415689	7	NULL	NULL	0	NULL	early surgical intervention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Traumatic coronary artery-cameral fistulas ( TCAF ) are uncommon sequelae of trauma that require early surgical intervention to prevent complications .
	manualset3
192551	5	415689	7	NULL	NULL	0	NULL	complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Traumatic coronary artery-cameral fistulas ( TCAF ) are uncommon sequelae of trauma that require early surgical intervention to prevent complications .
	manualset3
192552	1	415690	7	NULL	NULL	0	NULL	infusion 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After infusion of 0.4 micrograms/kg dDAVP , a 57-yr-old male patient had no increase in plasma factor VIII coagulant , ristocetin cofactor , or fibrinolytic activity or change in von Willebrand factor multimers .
	manualset3
192553	2	415690	7	NULL	NULL	0	NULL	0.4 micrograms/kg dDAVP	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	After infusion of 0.4 micrograms/kg dDAVP , a 57-yr-old male patient had no increase in plasma factor VIII coagulant , ristocetin cofactor , or fibrinolytic activity or change in von Willebrand factor multimers .
	manualset3
192554	3	415690	7	NULL	NULL	0	NULL	57-yr-old male patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	After infusion of 0.4 micrograms/kg dDAVP , a 57-yr-old male patient had no increase in plasma factor VIII coagulant , ristocetin cofactor , or fibrinolytic activity or change in von Willebrand factor multimers .
	manualset3
192555	4	415690	7	NULL	NULL	0	NULL	 plasma factor VIII coagulant	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	After infusion of 0.4 micrograms/kg dDAVP , a 57-yr-old male patient had no increase in plasma factor VIII coagulant , ristocetin cofactor , or fibrinolytic activity or change in von Willebrand factor multimers .
	manualset3
192556	5	415690	7	NULL	NULL	0	NULL	ristocetin cofactor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	After infusion of 0.4 micrograms/kg dDAVP , a 57-yr-old male patient had no increase in plasma factor VIII coagulant , ristocetin cofactor , or fibrinolytic activity or change in von Willebrand factor multimers .
	manualset3
192557	6	415690	7	NULL	NULL	0	NULL	fibrinolytic activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After infusion of 0.4 micrograms/kg dDAVP , a 57-yr-old male patient had no increase in plasma factor VIII coagulant , ristocetin cofactor , or fibrinolytic activity or change in von Willebrand factor multimers .
	manualset3
192558	7	415690	7	NULL	NULL	0	NULL	change 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After infusion of 0.4 micrograms/kg dDAVP , a 57-yr-old male patient had no increase in plasma factor VIII coagulant , ristocetin cofactor , or fibrinolytic activity or change in von Willebrand factor multimers .
	manualset3
192559	8	415690	7	NULL	NULL	0	NULL	von Willebrand factor multimers	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	After infusion of 0.4 micrograms/kg dDAVP , a 57-yr-old male patient had no increase in plasma factor VIII coagulant , ristocetin cofactor , or fibrinolytic activity or change in von Willebrand factor multimers .
	manualset3
192560	9	415690	7	NULL	NULL	0	NULL	increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After infusion of 0.4 micrograms/kg dDAVP , a 57-yr-old male patient had no increase in plasma factor VIII coagulant , ristocetin cofactor , or fibrinolytic activity or change in von Willebrand factor multimers .
	manualset3
192561	1	415691	7	NULL	NULL	0	NULL	Traumatic hyphema	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Traumatic hyphema can mimic increased intracranial pressure .
	manualset3
192562	2	415691	7	NULL	NULL	0	NULL	 increased intracranial pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Traumatic hyphema can mimic increased intracranial pressure .
	manualset3
192563	1	415692	7	NULL	NULL	0	NULL	Traumatic injuries	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Traumatic injuries involving the foot and ankle are very common .
	manualset3
192564	2	415692	7	NULL	NULL	0	NULL	foot and ankle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Traumatic injuries involving the foot and ankle are very common .
	manualset3
192565	1	415693	7	NULL	NULL	0	NULL	Travel times	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Travel times and radiotherapy uptake in two English counties .
	manualset3
192566	2	415693	7	NULL	NULL	0	NULL	radiotherapy uptake	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Travel times and radiotherapy uptake in two English counties .
	manualset3
192567	3	415693	7	NULL	NULL	0	NULL	two English counties	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Travel times and radiotherapy uptake in two English counties .
	manualset3
192568	1	415694	7	NULL	NULL	0	NULL	Treated solutions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treated solutions designed to simulate typical concentrations in dairy manure lagoon water , contained initial concentrations of urea up to 750 ppm ( mg L ( -1 ) ) , chloride from 100 to 400 ppm , and 2000 ppm NaHCO ( 3 ) .
	manualset3
192569	2	415694	7	NULL	NULL	0	NULL	typical concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treated solutions designed to simulate typical concentrations in dairy manure lagoon water , contained initial concentrations of urea up to 750 ppm ( mg L ( -1 ) ) , chloride from 100 to 400 ppm , and 2000 ppm NaHCO ( 3 ) .
	manualset3
192570	3	415694	7	NULL	NULL	0	NULL	dairy manure lagoon water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treated solutions designed to simulate typical concentrations in dairy manure lagoon water , contained initial concentrations of urea up to 750 ppm ( mg L ( -1 ) ) , chloride from 100 to 400 ppm , and 2000 ppm NaHCO ( 3 ) .
	manualset3
192571	4	415694	7	NULL	NULL	0	NULL	initial concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treated solutions designed to simulate typical concentrations in dairy manure lagoon water , contained initial concentrations of urea up to 750 ppm ( mg L ( -1 ) ) , chloride from 100 to 400 ppm , and 2000 ppm NaHCO ( 3 ) .
	manualset3
192572	5	415694	7	NULL	NULL	0	NULL	 urea	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treated solutions designed to simulate typical concentrations in dairy manure lagoon water , contained initial concentrations of urea up to 750 ppm ( mg L ( -1 ) ) , chloride from 100 to 400 ppm , and 2000 ppm NaHCO ( 3 ) .
	manualset3
192573	6	415694	7	NULL	NULL	0	NULL	750 ppm ( mg L ( -1 ) )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Treated solutions designed to simulate typical concentrations in dairy manure lagoon water , contained initial concentrations of urea up to 750 ppm ( mg L ( -1 ) ) , chloride from 100 to 400 ppm , and 2000 ppm NaHCO ( 3 ) .
	manualset3
192574	7	415694	7	NULL	NULL	0	NULL	chloride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treated solutions designed to simulate typical concentrations in dairy manure lagoon water , contained initial concentrations of urea up to 750 ppm ( mg L ( -1 ) ) , chloride from 100 to 400 ppm , and 2000 ppm NaHCO ( 3 ) .
	manualset3
192575	8	415694	7	NULL	NULL	0	NULL	100 ppm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Treated solutions designed to simulate typical concentrations in dairy manure lagoon water , contained initial concentrations of urea up to 750 ppm ( mg L ( -1 ) ) , chloride from 100 to 400 ppm , and 2000 ppm NaHCO ( 3 ) .
	manualset3
192576	9	415694	7	NULL	NULL	0	NULL	 400 ppm 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Treated solutions designed to simulate typical concentrations in dairy manure lagoon water , contained initial concentrations of urea up to 750 ppm ( mg L ( -1 ) ) , chloride from 100 to 400 ppm , and 2000 ppm NaHCO ( 3 ) .
	manualset3
192577	10	415694	7	NULL	NULL	0	NULL	2000 ppm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Treated solutions designed to simulate typical concentrations in dairy manure lagoon water , contained initial concentrations of urea up to 750 ppm ( mg L ( -1 ) ) , chloride from 100 to 400 ppm , and 2000 ppm NaHCO ( 3 ) .
	manualset3
192578	11	415694	7	NULL	NULL	0	NULL	NaHCO ( 3 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treated solutions designed to simulate typical concentrations in dairy manure lagoon water , contained initial concentrations of urea up to 750 ppm ( mg L ( -1 ) ) , chloride from 100 to 400 ppm , and 2000 ppm NaHCO ( 3 ) .
	manualset3
192579	1	415695	7	NULL	NULL	0	NULL	Treated wastewater 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treated wastewater is being increasingly used for irrigation and aquifer replenishment through artificial recharge .
	manualset3
192580	2	415695	7	NULL	NULL	0	NULL	irrigation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Treated wastewater is being increasingly used for irrigation and aquifer replenishment through artificial recharge .
	manualset3
192581	3	415695	7	NULL	NULL	0	NULL	aquifer replenishment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Treated wastewater is being increasingly used for irrigation and aquifer replenishment through artificial recharge .
	manualset3
192582	4	415695	7	NULL	NULL	0	NULL	artificial recharge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Treated wastewater is being increasingly used for irrigation and aquifer replenishment through artificial recharge .
	manualset3
192583	1	415696	7	NULL	NULL	0	NULL	metastatic solid tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Treating metastatic solid tumors with bortezomib and a tumor necrosis factor-related apoptosis-inducing ligand receptor agonist antibody .
	manualset3
192584	2	415696	7	NULL	NULL	0	NULL	bortezomib	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Treating metastatic solid tumors with bortezomib and a tumor necrosis factor-related apoptosis-inducing ligand receptor agonist antibody .
	manualset3
192585	3	415696	7	NULL	NULL	0	NULL	tumor necrosis factor-related apoptosis-inducing ligand receptor agonist antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treating metastatic solid tumors with bortezomib and a tumor necrosis factor-related apoptosis-inducing ligand receptor agonist antibody .
	manualset3
192586	1	415697	7	NULL	NULL	0	NULL	Treating oppositional defiant disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Treating oppositional defiant disorder in primary care : a comparison of three models .
	manualset3
192587	2	415697	7	NULL	NULL	0	NULL	primary care	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Treating oppositional defiant disorder in primary care : a comparison of three models .
	manualset3
192588	3	415697	7	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Treating oppositional defiant disorder in primary care : a comparison of three models .
	manualset3
192589	4	415697	7	NULL	NULL	0	NULL	three models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Treating oppositional defiant disorder in primary care : a comparison of three models .
	manualset3
192590	1	415698	7	NULL	NULL	0	NULL	Treatment-emergent akathisia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment-emergent akathisia was not associated with a poorer clinical response .
	manualset3
192591	2	415698	7	NULL	NULL	0	NULL	 poorer clinical response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment-emergent akathisia was not associated with a poorer clinical response .
	manualset3
192592	1	415699	7	NULL	NULL	NULL	NULL	Treatment advancements	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Treatment advancements in MBC are not reflected by better survival for the whole MBC population .
	manualset3
192593	2	415699	7	NULL	NULL	0	NULL	MBC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment advancements in MBC are not reflected by better survival for the whole MBC population .
	manualset3
192594	3	415699	7	NULL	NULL	0	NULL	 survival 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment advancements in MBC are not reflected by better survival for the whole MBC population .
	manualset3
192595	4	415699	7	NULL	NULL	0	NULL	whole MBC population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment advancements in MBC are not reflected by better survival for the whole MBC population .
	manualset3
192596	1	415700	7	NULL	NULL	0	NULL	initial discrimination training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After initial discrimination training in which animals learned to press one lever after a 2-s tone duration , and the other lever after a 8-s tone duration for food reward , the bisection procedure was implemented in which intermediate durations with no available reinforcement were interspersed with trials with the anchor durations .
	manualset3
192597	2	415700	7	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	After initial discrimination training in which animals learned to press one lever after a 2-s tone duration , and the other lever after a 8-s tone duration for food reward , the bisection procedure was implemented in which intermediate durations with no available reinforcement were interspersed with trials with the anchor durations .
	manualset3
192598	3	415700	7	NULL	NULL	0	NULL	one lever	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	After initial discrimination training in which animals learned to press one lever after a 2-s tone duration , and the other lever after a 8-s tone duration for food reward , the bisection procedure was implemented in which intermediate durations with no available reinforcement were interspersed with trials with the anchor durations .
	manualset3
192599	4	415700	7	NULL	NULL	0	NULL	2-s tone duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After initial discrimination training in which animals learned to press one lever after a 2-s tone duration , and the other lever after a 8-s tone duration for food reward , the bisection procedure was implemented in which intermediate durations with no available reinforcement were interspersed with trials with the anchor durations .
	manualset3
192600	5	415700	7	NULL	NULL	0	NULL	 other lever	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	After initial discrimination training in which animals learned to press one lever after a 2-s tone duration , and the other lever after a 8-s tone duration for food reward , the bisection procedure was implemented in which intermediate durations with no available reinforcement were interspersed with trials with the anchor durations .
	manualset3
192601	6	415700	7	NULL	NULL	0	NULL	8-s tone duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After initial discrimination training in which animals learned to press one lever after a 2-s tone duration , and the other lever after a 8-s tone duration for food reward , the bisection procedure was implemented in which intermediate durations with no available reinforcement were interspersed with trials with the anchor durations .
	manualset3
192602	7	415700	7	NULL	NULL	0	NULL	food reward	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After initial discrimination training in which animals learned to press one lever after a 2-s tone duration , and the other lever after a 8-s tone duration for food reward , the bisection procedure was implemented in which intermediate durations with no available reinforcement were interspersed with trials with the anchor durations .
	manualset3
192603	8	415700	7	NULL	NULL	0	NULL	bisection procedure 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After initial discrimination training in which animals learned to press one lever after a 2-s tone duration , and the other lever after a 8-s tone duration for food reward , the bisection procedure was implemented in which intermediate durations with no available reinforcement were interspersed with trials with the anchor durations .
	manualset3
192604	9	415700	7	NULL	NULL	0	NULL	intermediate durations	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After initial discrimination training in which animals learned to press one lever after a 2-s tone duration , and the other lever after a 8-s tone duration for food reward , the bisection procedure was implemented in which intermediate durations with no available reinforcement were interspersed with trials with the anchor durations .
	manualset3
192605	10	415700	7	NULL	NULL	0	NULL	no available reinforcement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After initial discrimination training in which animals learned to press one lever after a 2-s tone duration , and the other lever after a 8-s tone duration for food reward , the bisection procedure was implemented in which intermediate durations with no available reinforcement were interspersed with trials with the anchor durations .
	manualset3
192606	11	415700	7	NULL	NULL	0	NULL	trials	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After initial discrimination training in which animals learned to press one lever after a 2-s tone duration , and the other lever after a 8-s tone duration for food reward , the bisection procedure was implemented in which intermediate durations with no available reinforcement were interspersed with trials with the anchor durations .
	manualset3
192607	12	415700	7	NULL	NULL	0	NULL	anchor durations	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After initial discrimination training in which animals learned to press one lever after a 2-s tone duration , and the other lever after a 8-s tone duration for food reward , the bisection procedure was implemented in which intermediate durations with no available reinforcement were interspersed with trials with the anchor durations .
	manualset3
192608	1	415701	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment at the time of injury resulted in significant decreases in onset-time and severity of pain behavior , while treatment at the time of onset led to a significant reduction of the spontaneous self-directed behavior .
	manualset3
192609	2	415701	7	NULL	NULL	0	NULL	time of injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment at the time of injury resulted in significant decreases in onset-time and severity of pain behavior , while treatment at the time of onset led to a significant reduction of the spontaneous self-directed behavior .
	manualset3
192610	3	415701	7	NULL	NULL	0	NULL	onset-time	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment at the time of injury resulted in significant decreases in onset-time and severity of pain behavior , while treatment at the time of onset led to a significant reduction of the spontaneous self-directed behavior .
	manualset3
192611	4	415701	7	NULL	NULL	0	NULL	severity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment at the time of injury resulted in significant decreases in onset-time and severity of pain behavior , while treatment at the time of onset led to a significant reduction of the spontaneous self-directed behavior .
	manualset3
192612	5	415701	7	NULL	NULL	0	NULL	pain behavior	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment at the time of injury resulted in significant decreases in onset-time and severity of pain behavior , while treatment at the time of onset led to a significant reduction of the spontaneous self-directed behavior .
	manualset3
192613	6	415701	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment at the time of injury resulted in significant decreases in onset-time and severity of pain behavior , while treatment at the time of onset led to a significant reduction of the spontaneous self-directed behavior .
	manualset3
192614	7	415701	7	NULL	NULL	0	NULL	time of onset	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment at the time of injury resulted in significant decreases in onset-time and severity of pain behavior , while treatment at the time of onset led to a significant reduction of the spontaneous self-directed behavior .
	manualset3
192615	8	415701	7	NULL	NULL	0	NULL	significant reduction	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment at the time of injury resulted in significant decreases in onset-time and severity of pain behavior , while treatment at the time of onset led to a significant reduction of the spontaneous self-directed behavior .
	manualset3
192616	9	415701	7	NULL	NULL	NULL	NULL	spontaneous self-directed behavior	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Treatment at the time of injury resulted in significant decreases in onset-time and severity of pain behavior , while treatment at the time of onset led to a significant reduction of the spontaneous self-directed behavior .
	manualset3
192617	1	415702	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment consisted of corticosteroids ( 32 patients ) , antimalarials ( 14 ) , cyclophosphamide ( 9 ) or azathioprine ( 2 ) .
	manualset3
192618	2	415702	7	NULL	NULL	NULL	NULL	corticosteroids	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Treatment consisted of corticosteroids ( 32 patients ) , antimalarials ( 14 ) , cyclophosphamide ( 9 ) or azathioprine ( 2 ) .
	manualset3
192619	3	415702	7	NULL	NULL	0	NULL	32 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment consisted of corticosteroids ( 32 patients ) , antimalarials ( 14 ) , cyclophosphamide ( 9 ) or azathioprine ( 2 ) .
	manualset3
192620	4	415702	7	NULL	NULL	0	NULL	antimalarials ( 14 )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment consisted of corticosteroids ( 32 patients ) , antimalarials ( 14 ) , cyclophosphamide ( 9 ) or azathioprine ( 2 ) .
	manualset3
192621	5	415702	7	NULL	NULL	0	NULL	cyclophosphamide ( 9 )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment consisted of corticosteroids ( 32 patients ) , antimalarials ( 14 ) , cyclophosphamide ( 9 ) or azathioprine ( 2 ) .
	manualset3
192622	6	415702	7	NULL	NULL	0	NULL	azathioprine ( 2 )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment consisted of corticosteroids ( 32 patients ) , antimalarials ( 14 ) , cyclophosphamide ( 9 ) or azathioprine ( 2 ) .
	manualset3
192623	1	415703	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment consisted of radiation therapy and intrathecal chemotherapy with arabinoside-cytosine and systemic chemotherapy .
	manualset3
192624	2	415703	7	NULL	NULL	0	NULL	radiation therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment consisted of radiation therapy and intrathecal chemotherapy with arabinoside-cytosine and systemic chemotherapy .
	manualset3
192625	3	415703	7	NULL	NULL	0	NULL	intrathecal chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment consisted of radiation therapy and intrathecal chemotherapy with arabinoside-cytosine and systemic chemotherapy .
	manualset3
192626	4	415703	7	NULL	NULL	0	NULL	arabinoside-cytosine chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment consisted of radiation therapy and intrathecal chemotherapy with arabinoside-cytosine and systemic chemotherapy .
	manualset3
192627	5	415703	7	NULL	NULL	0	NULL	systemic chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment consisted of radiation therapy and intrathecal chemotherapy with arabinoside-cytosine and systemic chemotherapy .
	manualset3
192628	1	415704	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment effect may be enhanced among patients undergoing early coronary revascularization , with evidence of stabilization before intervention and suppression of postprocedural ischemic events .
	manualset3
192629	2	415704	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment effect may be enhanced among patients undergoing early coronary revascularization , with evidence of stabilization before intervention and suppression of postprocedural ischemic events .
	manualset3
192630	3	415704	7	NULL	NULL	0	NULL	early coronary revascularization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment effect may be enhanced among patients undergoing early coronary revascularization , with evidence of stabilization before intervention and suppression of postprocedural ischemic events .
	manualset3
192631	4	415704	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment effect may be enhanced among patients undergoing early coronary revascularization , with evidence of stabilization before intervention and suppression of postprocedural ischemic events .
	manualset3
192632	5	415704	7	NULL	NULL	0	NULL	 stabilization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment effect may be enhanced among patients undergoing early coronary revascularization , with evidence of stabilization before intervention and suppression of postprocedural ischemic events .
	manualset3
192633	6	415704	7	NULL	NULL	0	NULL	 intervention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment effect may be enhanced among patients undergoing early coronary revascularization , with evidence of stabilization before intervention and suppression of postprocedural ischemic events .
	manualset3
192634	7	415704	7	NULL	NULL	0	NULL	suppression	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment effect may be enhanced among patients undergoing early coronary revascularization , with evidence of stabilization before intervention and suppression of postprocedural ischemic events .
	manualset3
192635	8	415704	7	NULL	NULL	0	NULL	postprocedural ischemic events	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment effect may be enhanced among patients undergoing early coronary revascularization , with evidence of stabilization before intervention and suppression of postprocedural ischemic events .
	manualset3
192636	1	415705	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of AcMCP 1-infected Sf-21 cells with tunicamycin resulted in reduced production of the 21 - and 23-kDa proteins and an increase in 16 - to 18-kDa products , the predicted size range of uncleaved and nonglycosylated rat MCP 1 .
	manualset3
192637	2	415705	7	NULL	NULL	0	NULL	AcMCP 1-infected Sf-21 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of AcMCP 1-infected Sf-21 cells with tunicamycin resulted in reduced production of the 21 - and 23-kDa proteins and an increase in 16 - to 18-kDa products , the predicted size range of uncleaved and nonglycosylated rat MCP 1 .
	manualset3
192638	3	415705	7	NULL	NULL	0	NULL	tunicamycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of AcMCP 1-infected Sf-21 cells with tunicamycin resulted in reduced production of the 21 - and 23-kDa proteins and an increase in 16 - to 18-kDa products , the predicted size range of uncleaved and nonglycosylated rat MCP 1 .
	manualset3
192639	4	415705	7	NULL	NULL	0	NULL	reduced production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of AcMCP 1-infected Sf-21 cells with tunicamycin resulted in reduced production of the 21 - and 23-kDa proteins and an increase in 16 - to 18-kDa products , the predicted size range of uncleaved and nonglycosylated rat MCP 1 .
	manualset3
192640	5	415705	7	NULL	NULL	NULL	NULL	21-kDa proteins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Treatment of AcMCP 1-infected Sf-21 cells with tunicamycin resulted in reduced production of the 21 - and 23-kDa proteins and an increase in 16 - to 18-kDa products , the predicted size range of uncleaved and nonglycosylated rat MCP 1 .
	manualset3
192641	6	415705	7	NULL	NULL	NULL	NULL	23-kDa proteins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Treatment of AcMCP 1-infected Sf-21 cells with tunicamycin resulted in reduced production of the 21 - and 23-kDa proteins and an increase in 16 - to 18-kDa products , the predicted size range of uncleaved and nonglycosylated rat MCP 1 .
	manualset3
192642	7	415705	7	NULL	NULL	0	NULL	increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of AcMCP 1-infected Sf-21 cells with tunicamycin resulted in reduced production of the 21 - and 23-kDa proteins and an increase in 16 - to 18-kDa products , the predicted size range of uncleaved and nonglycosylated rat MCP 1 .
	manualset3
192643	8	415705	7	NULL	NULL	NULL	NULL	16 -kDa products	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Treatment of AcMCP 1-infected Sf-21 cells with tunicamycin resulted in reduced production of the 21 - and 23-kDa proteins and an increase in 16 - to 18-kDa products , the predicted size range of uncleaved and nonglycosylated rat MCP 1 .
	manualset3
192644	9	415705	7	NULL	NULL	NULL	NULL	18-kDa products	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Treatment of AcMCP 1-infected Sf-21 cells with tunicamycin resulted in reduced production of the 21 - and 23-kDa proteins and an increase in 16 - to 18-kDa products , the predicted size range of uncleaved and nonglycosylated rat MCP 1 .
	manualset3
192645	10	415705	7	NULL	NULL	0	NULL	predicted size range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of AcMCP 1-infected Sf-21 cells with tunicamycin resulted in reduced production of the 21 - and 23-kDa proteins and an increase in 16 - to 18-kDa products , the predicted size range of uncleaved and nonglycosylated rat MCP 1 .
	manualset3
192646	11	415705	7	NULL	NULL	0	NULL	uncleaved and nonglycosylated rat MCP 1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of AcMCP 1-infected Sf-21 cells with tunicamycin resulted in reduced production of the 21 - and 23-kDa proteins and an increase in 16 - to 18-kDa products , the predicted size range of uncleaved and nonglycosylated rat MCP 1 .
	manualset3
192647	1	415706	7	NULL	NULL	0	NULL	Treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of CaCo2-3B with the alpha ( 2 ) - adrenoreceptor agonist 5-bromo-6 - ( 2-imidazolin-2-ylamino ) quinoxaline ( UK14304 ) induces not only ERK , but also Akt phosphorylation .
	manualset3
192648	2	415706	7	NULL	NULL	0	NULL	CaCo2-3B 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of CaCo2-3B with the alpha ( 2 ) - adrenoreceptor agonist 5-bromo-6 - ( 2-imidazolin-2-ylamino ) quinoxaline ( UK14304 ) induces not only ERK , but also Akt phosphorylation .
	manualset3
192649	3	415706	7	NULL	NULL	0	NULL	alpha ( 2 ) - adrenoreceptor agonist 5-bromo-6 - ( 2-imidazolin-2-ylamino ) quinoxaline ( UK14304 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of CaCo2-3B with the alpha ( 2 ) - adrenoreceptor agonist 5-bromo-6 - ( 2-imidazolin-2-ylamino ) quinoxaline ( UK14304 ) induces not only ERK , but also Akt phosphorylation .
	manualset3
192650	4	415706	7	NULL	NULL	0	NULL	ERK 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of CaCo2-3B with the alpha ( 2 ) - adrenoreceptor agonist 5-bromo-6 - ( 2-imidazolin-2-ylamino ) quinoxaline ( UK14304 ) induces not only ERK , but also Akt phosphorylation .
	manualset3
192651	5	415706	7	NULL	NULL	0	NULL	Akt phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of CaCo2-3B with the alpha ( 2 ) - adrenoreceptor agonist 5-bromo-6 - ( 2-imidazolin-2-ylamino ) quinoxaline ( UK14304 ) induces not only ERK , but also Akt phosphorylation .
	manualset3
192652	1	415707	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of Cr ( VI ) - containing wastewaters with exopolysaccharide-producing cyanobacteria in pilot flow through and batch systems .
	manualset3
192653	2	415707	7	NULL	NULL	0	NULL	Cr ( VI ) - containing wastewaters	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of Cr ( VI ) - containing wastewaters with exopolysaccharide-producing cyanobacteria in pilot flow through and batch systems .
	manualset3
192654	3	415707	7	NULL	NULL	0	NULL	exopolysaccharide-producing cyanobacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of Cr ( VI ) - containing wastewaters with exopolysaccharide-producing cyanobacteria in pilot flow through and batch systems .
	manualset3
192655	4	415707	7	NULL	NULL	0	NULL	pilot flow	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of Cr ( VI ) - containing wastewaters with exopolysaccharide-producing cyanobacteria in pilot flow through and batch systems .
	manualset3
192656	5	415707	7	NULL	NULL	0	NULL	batch systems 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of Cr ( VI ) - containing wastewaters with exopolysaccharide-producing cyanobacteria in pilot flow through and batch systems .
	manualset3
192657	1	415708	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of T4-2 breast cancer cells in three-dimensional culture with cAMP analogs or a phosphatidylinositol 3-kinase inhibitor not only reverted their phenotype from nonpolar to polar acinar-like structures but also enhanced chromatin sensitivity to AluI .
	manualset3
192658	2	415708	7	NULL	NULL	0	NULL	T4-2 breast cancer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of T4-2 breast cancer cells in three-dimensional culture with cAMP analogs or a phosphatidylinositol 3-kinase inhibitor not only reverted their phenotype from nonpolar to polar acinar-like structures but also enhanced chromatin sensitivity to AluI .
	manualset3
192659	3	415708	7	NULL	NULL	0	NULL	three-dimensional culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of T4-2 breast cancer cells in three-dimensional culture with cAMP analogs or a phosphatidylinositol 3-kinase inhibitor not only reverted their phenotype from nonpolar to polar acinar-like structures but also enhanced chromatin sensitivity to AluI .
	manualset3
192660	4	415708	7	NULL	NULL	0	NULL	cAMP analogs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of T4-2 breast cancer cells in three-dimensional culture with cAMP analogs or a phosphatidylinositol 3-kinase inhibitor not only reverted their phenotype from nonpolar to polar acinar-like structures but also enhanced chromatin sensitivity to AluI .
	manualset3
192661	5	415708	7	NULL	NULL	0	NULL	phosphatidylinositol 3-kinase inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of T4-2 breast cancer cells in three-dimensional culture with cAMP analogs or a phosphatidylinositol 3-kinase inhibitor not only reverted their phenotype from nonpolar to polar acinar-like structures but also enhanced chromatin sensitivity to AluI .
	manualset3
192662	6	415708	7	NULL	NULL	0	NULL	phenotype	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of T4-2 breast cancer cells in three-dimensional culture with cAMP analogs or a phosphatidylinositol 3-kinase inhibitor not only reverted their phenotype from nonpolar to polar acinar-like structures but also enhanced chromatin sensitivity to AluI .
	manualset3
192663	7	415708	7	NULL	NULL	0	NULL	nonpolar acinar-like structures 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of T4-2 breast cancer cells in three-dimensional culture with cAMP analogs or a phosphatidylinositol 3-kinase inhibitor not only reverted their phenotype from nonpolar to polar acinar-like structures but also enhanced chromatin sensitivity to AluI .
	manualset3
192664	8	415708	7	NULL	NULL	0	NULL	polar acinar-like structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of T4-2 breast cancer cells in three-dimensional culture with cAMP analogs or a phosphatidylinositol 3-kinase inhibitor not only reverted their phenotype from nonpolar to polar acinar-like structures but also enhanced chromatin sensitivity to AluI .
	manualset3
192665	9	415708	7	NULL	NULL	0	NULL	enhanced chromatin sensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of T4-2 breast cancer cells in three-dimensional culture with cAMP analogs or a phosphatidylinositol 3-kinase inhibitor not only reverted their phenotype from nonpolar to polar acinar-like structures but also enhanced chromatin sensitivity to AluI .
	manualset3
192666	10	415708	7	NULL	NULL	0	NULL	AluI	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of T4-2 breast cancer cells in three-dimensional culture with cAMP analogs or a phosphatidylinositol 3-kinase inhibitor not only reverted their phenotype from nonpolar to polar acinar-like structures but also enhanced chromatin sensitivity to AluI .
	manualset3
192667	1	415709	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of acute infections in the upper airways comprises a significant part of direct healthcare expenditure and is a challenge for healthcare professionals .
	manualset3
192668	2	415709	7	NULL	NULL	0	NULL	acute infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of acute infections in the upper airways comprises a significant part of direct healthcare expenditure and is a challenge for healthcare professionals .
	manualset3
192669	3	415709	7	NULL	NULL	0	NULL	upper airways	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of acute infections in the upper airways comprises a significant part of direct healthcare expenditure and is a challenge for healthcare professionals .
	manualset3
192670	4	415709	7	NULL	NULL	0	NULL	direct healthcare expenditure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of acute infections in the upper airways comprises a significant part of direct healthcare expenditure and is a challenge for healthcare professionals .
	manualset3
192671	5	415709	7	NULL	NULL	0	NULL	healthcare professionals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of acute infections in the upper airways comprises a significant part of direct healthcare expenditure and is a challenge for healthcare professionals .
	manualset3
192672	1	415710	7	NULL	NULL	0	NULL	Treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of acute renal transplant rejection with FK 506 in patients on cyclosporine after failure of standard antirejection therapy .
	manualset3
192673	2	415710	7	NULL	NULL	0	NULL	acute renal transplant rejection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of acute renal transplant rejection with FK 506 in patients on cyclosporine after failure of standard antirejection therapy .
	manualset3
192674	3	415710	7	NULL	NULL	0	NULL	FK 506	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of acute renal transplant rejection with FK 506 in patients on cyclosporine after failure of standard antirejection therapy .
	manualset3
192675	4	415710	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of acute renal transplant rejection with FK 506 in patients on cyclosporine after failure of standard antirejection therapy .
	manualset3
192676	5	415710	7	NULL	NULL	0	NULL	cyclosporine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of acute renal transplant rejection with FK 506 in patients on cyclosporine after failure of standard antirejection therapy .
	manualset3
192677	6	415710	7	NULL	NULL	0	NULL	failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of acute renal transplant rejection with FK 506 in patients on cyclosporine after failure of standard antirejection therapy .
	manualset3
192678	7	415710	7	NULL	NULL	0	NULL	standard antirejection therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of acute renal transplant rejection with FK 506 in patients on cyclosporine after failure of standard antirejection therapy .
	manualset3
192679	1	415711	7	NULL	NULL	0	NULL	Treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of agitation and aggression in bipolar mania : efficacy of quetiapine .
	manualset3
192680	2	415711	7	NULL	NULL	0	NULL	agitation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of agitation and aggression in bipolar mania : efficacy of quetiapine .
	manualset3
192681	3	415711	7	NULL	NULL	0	NULL	aggression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of agitation and aggression in bipolar mania : efficacy of quetiapine .
	manualset3
192682	4	415711	7	NULL	NULL	0	NULL	 bipolar mania	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of agitation and aggression in bipolar mania : efficacy of quetiapine .
	manualset3
192683	5	415711	7	NULL	NULL	0	NULL	efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of agitation and aggression in bipolar mania : efficacy of quetiapine .
	manualset3
192684	6	415711	7	NULL	NULL	0	NULL	quetiapine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of agitation and aggression in bipolar mania : efficacy of quetiapine .
	manualset3
192685	1	415712	7	NULL	NULL	0	NULL	Treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of animals with 500 mg/kg GO resulted in suppression of P4502E1-mediated catalytic activities , as monitored by both PNP and aniline hydroxylase activities , whereas the effects at the dose of 1000 mg/kg were identical with those at 500 mg/kg b.w. 3 .
	manualset3
192686	2	415712	7	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of animals with 500 mg/kg GO resulted in suppression of P4502E1-mediated catalytic activities , as monitored by both PNP and aniline hydroxylase activities , whereas the effects at the dose of 1000 mg/kg were identical with those at 500 mg/kg b.w. 3 .
	manualset3
192687	3	415712	7	NULL	NULL	0	NULL	500 mg/kg	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of animals with 500 mg/kg GO resulted in suppression of P4502E1-mediated catalytic activities , as monitored by both PNP and aniline hydroxylase activities , whereas the effects at the dose of 1000 mg/kg were identical with those at 500 mg/kg b.w. 3 .
	manualset3
192688	4	415712	7	NULL	NULL	0	NULL	GO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of animals with 500 mg/kg GO resulted in suppression of P4502E1-mediated catalytic activities , as monitored by both PNP and aniline hydroxylase activities , whereas the effects at the dose of 1000 mg/kg were identical with those at 500 mg/kg b.w. 3 .
	manualset3
192689	5	415712	7	NULL	NULL	0	NULL	suppression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of animals with 500 mg/kg GO resulted in suppression of P4502E1-mediated catalytic activities , as monitored by both PNP and aniline hydroxylase activities , whereas the effects at the dose of 1000 mg/kg were identical with those at 500 mg/kg b.w. 3 .
	manualset3
192690	6	415712	7	NULL	NULL	0	NULL	P4502E1-mediated catalytic activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of animals with 500 mg/kg GO resulted in suppression of P4502E1-mediated catalytic activities , as monitored by both PNP and aniline hydroxylase activities , whereas the effects at the dose of 1000 mg/kg were identical with those at 500 mg/kg b.w. 3 .
	manualset3
192691	7	415712	7	NULL	NULL	0	NULL	PNP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of animals with 500 mg/kg GO resulted in suppression of P4502E1-mediated catalytic activities , as monitored by both PNP and aniline hydroxylase activities , whereas the effects at the dose of 1000 mg/kg were identical with those at 500 mg/kg b.w. 3 .
	manualset3
192692	8	415712	7	NULL	NULL	0	NULL	aniline hydroxylase activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of animals with 500 mg/kg GO resulted in suppression of P4502E1-mediated catalytic activities , as monitored by both PNP and aniline hydroxylase activities , whereas the effects at the dose of 1000 mg/kg were identical with those at 500 mg/kg b.w. 3 .
	manualset3
192693	9	415712	7	NULL	NULL	0	NULL	effects 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of animals with 500 mg/kg GO resulted in suppression of P4502E1-mediated catalytic activities , as monitored by both PNP and aniline hydroxylase activities , whereas the effects at the dose of 1000 mg/kg were identical with those at 500 mg/kg b.w. 3 .
	manualset3
192694	10	415712	7	NULL	NULL	0	NULL	dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of animals with 500 mg/kg GO resulted in suppression of P4502E1-mediated catalytic activities , as monitored by both PNP and aniline hydroxylase activities , whereas the effects at the dose of 1000 mg/kg were identical with those at 500 mg/kg b.w. 3 .
	manualset3
192695	11	415712	7	NULL	NULL	0	NULL	1000 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of animals with 500 mg/kg GO resulted in suppression of P4502E1-mediated catalytic activities , as monitored by both PNP and aniline hydroxylase activities , whereas the effects at the dose of 1000 mg/kg were identical with those at 500 mg/kg b.w. 3 .
	manualset3
192696	12	415712	7	NULL	NULL	0	NULL	500 mg/kg b.w. 3	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of animals with 500 mg/kg GO resulted in suppression of P4502E1-mediated catalytic activities , as monitored by both PNP and aniline hydroxylase activities , whereas the effects at the dose of 1000 mg/kg were identical with those at 500 mg/kg b.w. 3 .
	manualset3
192697	1	415713	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of cells with fangchinoline significantly inhibited MDA-MB-231 cell proliferation in a concentration - and time-dependent manner .
	manualset3
192698	2	415713	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of cells with fangchinoline significantly inhibited MDA-MB-231 cell proliferation in a concentration - and time-dependent manner .
	manualset3
192699	3	415713	7	NULL	NULL	0	NULL	fangchinoline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of cells with fangchinoline significantly inhibited MDA-MB-231 cell proliferation in a concentration - and time-dependent manner .
	manualset3
192700	4	415713	7	NULL	NULL	0	NULL	MDA-MB-231 cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of cells with fangchinoline significantly inhibited MDA-MB-231 cell proliferation in a concentration - and time-dependent manner .
	manualset3
192701	5	415713	7	NULL	NULL	0	NULL	concentration -dependent manner	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of cells with fangchinoline significantly inhibited MDA-MB-231 cell proliferation in a concentration - and time-dependent manner .
	manualset3
192702	6	415713	7	NULL	NULL	0	NULL	time-dependent manner	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of cells with fangchinoline significantly inhibited MDA-MB-231 cell proliferation in a concentration - and time-dependent manner .
	manualset3
192703	1	415714	7	NULL	NULL	0	NULL	Treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of children for primary acute herpetic gingivostomatitis with lactobacillus in aqueous suspension .
	manualset3
192704	2	415714	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of children for primary acute herpetic gingivostomatitis with lactobacillus in aqueous suspension .
	manualset3
192705	3	415714	7	NULL	NULL	0	NULL	primary acute herpetic gingivostomatitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of children for primary acute herpetic gingivostomatitis with lactobacillus in aqueous suspension .
	manualset3
192706	4	415714	7	NULL	NULL	0	NULL	 lactobacillus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of children for primary acute herpetic gingivostomatitis with lactobacillus in aqueous suspension .
	manualset3
192707	5	415714	7	NULL	NULL	0	NULL	aqueous suspension	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of children for primary acute herpetic gingivostomatitis with lactobacillus in aqueous suspension .
	manualset3
192708	1	415715	7	NULL	NULL	0	NULL	Treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of cisplatin resulted in ROS generation and lipid peroxidation in HEI-OC1 .
	manualset3
192709	2	415715	7	NULL	NULL	0	NULL	cisplatin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of cisplatin resulted in ROS generation and lipid peroxidation in HEI-OC1 .
	manualset3
192710	3	415715	7	NULL	NULL	0	NULL	ROS generation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of cisplatin resulted in ROS generation and lipid peroxidation in HEI-OC1 .
	manualset3
192711	4	415715	7	NULL	NULL	0	NULL	lipid peroxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of cisplatin resulted in ROS generation and lipid peroxidation in HEI-OC1 .
	manualset3
192712	5	415715	7	NULL	NULL	0	NULL	HEI-OC1	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of cisplatin resulted in ROS generation and lipid peroxidation in HEI-OC1 .
	manualset3
192810	1	415716	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of deep vein thrombosis with low-molecular-weight heparins : a consensus statement of the Gesellschaft fr Thrombose-und Hmostaseforschung ( GTH ) .
	manualset3
192811	2	415716	7	NULL	NULL	0	NULL	deep vein thrombosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of deep vein thrombosis with low-molecular-weight heparins : a consensus statement of the Gesellschaft fr Thrombose-und Hmostaseforschung ( GTH ) .
	manualset3
192812	3	415716	7	NULL	NULL	0	NULL	 low-molecular-weight heparins	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of deep vein thrombosis with low-molecular-weight heparins : a consensus statement of the Gesellschaft fr Thrombose-und Hmostaseforschung ( GTH ) .
	manualset3
192813	4	415716	7	NULL	NULL	0	NULL	consensus statement 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of deep vein thrombosis with low-molecular-weight heparins : a consensus statement of the Gesellschaft fr Thrombose-und Hmostaseforschung ( GTH ) .
	manualset3
192814	5	415716	7	NULL	NULL	0	NULL	Gesellschaft fr Thrombose-und Hmostaseforschung ( GTH )	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of deep vein thrombosis with low-molecular-weight heparins : a consensus statement of the Gesellschaft fr Thrombose-und Hmostaseforschung ( GTH ) .
	manualset3
192815	1	415717	7	NULL	NULL	0	NULL	 injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After injection into rat myocardium , biotinylated nanofibers provided sustained IGF-1 delivery for 28 days , and targeted delivery of IGF-1 in vivo increased activation of Akt in the myocardium .
	manualset3
192816	2	415717	7	NULL	NULL	0	NULL	rat myocardium 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After injection into rat myocardium , biotinylated nanofibers provided sustained IGF-1 delivery for 28 days , and targeted delivery of IGF-1 in vivo increased activation of Akt in the myocardium .
	manualset3
192817	3	415717	7	NULL	NULL	0	NULL	biotinylated nanofibers	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	After injection into rat myocardium , biotinylated nanofibers provided sustained IGF-1 delivery for 28 days , and targeted delivery of IGF-1 in vivo increased activation of Akt in the myocardium .
	manualset3
192818	4	415717	7	NULL	NULL	0	NULL	sustained IGF-1 delivery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After injection into rat myocardium , biotinylated nanofibers provided sustained IGF-1 delivery for 28 days , and targeted delivery of IGF-1 in vivo increased activation of Akt in the myocardium .
	manualset3
192819	5	415717	7	NULL	NULL	0	NULL	 28 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After injection into rat myocardium , biotinylated nanofibers provided sustained IGF-1 delivery for 28 days , and targeted delivery of IGF-1 in vivo increased activation of Akt in the myocardium .
	manualset3
192820	6	415717	7	NULL	NULL	0	NULL	targeted delivery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After injection into rat myocardium , biotinylated nanofibers provided sustained IGF-1 delivery for 28 days , and targeted delivery of IGF-1 in vivo increased activation of Akt in the myocardium .
	manualset3
192821	7	415717	7	NULL	NULL	0	NULL	IGF-1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	After injection into rat myocardium , biotinylated nanofibers provided sustained IGF-1 delivery for 28 days , and targeted delivery of IGF-1 in vivo increased activation of Akt in the myocardium .
	manualset3
192822	8	415717	7	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After injection into rat myocardium , biotinylated nanofibers provided sustained IGF-1 delivery for 28 days , and targeted delivery of IGF-1 in vivo increased activation of Akt in the myocardium .
	manualset3
192823	9	415717	7	NULL	NULL	0	NULL	Akt	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	After injection into rat myocardium , biotinylated nanofibers provided sustained IGF-1 delivery for 28 days , and targeted delivery of IGF-1 in vivo increased activation of Akt in the myocardium .
	manualset3
192824	10	415717	7	NULL	NULL	0	NULL	myocardium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After injection into rat myocardium , biotinylated nanofibers provided sustained IGF-1 delivery for 28 days , and targeted delivery of IGF-1 in vivo increased activation of Akt in the myocardium .
	manualset3
192825	1	415718	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of displaced supracondylar fractures of the humerus in children by a pin leverage technique .
	manualset3
192826	2	415718	7	NULL	NULL	0	NULL	displaced supracondylar fractures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of displaced supracondylar fractures of the humerus in children by a pin leverage technique .
	manualset3
192827	3	415718	7	NULL	NULL	0	NULL	humerus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of displaced supracondylar fractures of the humerus in children by a pin leverage technique .
	manualset3
192828	4	415718	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of displaced supracondylar fractures of the humerus in children by a pin leverage technique .
	manualset3
192829	5	415718	7	NULL	NULL	0	NULL	pin leverage technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of displaced supracondylar fractures of the humerus in children by a pin leverage technique .
	manualset3
192830	1	415719	7	NULL	NULL	0	NULL	Treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of electronic waste to recover metal values using thermal plasma coupled with acid leaching -- a response surface modeling approach .
	manualset3
192831	2	415719	7	NULL	NULL	0	NULL	electronic waste 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of electronic waste to recover metal values using thermal plasma coupled with acid leaching -- a response surface modeling approach .
	manualset3
192832	3	415719	7	NULL	NULL	0	NULL	metal values	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of electronic waste to recover metal values using thermal plasma coupled with acid leaching -- a response surface modeling approach .
	manualset3
192833	4	415719	7	NULL	NULL	0	NULL	thermal plasma coupled with acid leaching	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of electronic waste to recover metal values using thermal plasma coupled with acid leaching -- a response surface modeling approach .
	manualset3
192834	5	415719	7	NULL	NULL	0	NULL	response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of electronic waste to recover metal values using thermal plasma coupled with acid leaching -- a response surface modeling approach .
	manualset3
192835	6	415719	7	NULL	NULL	0	NULL	surface modeling approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of electronic waste to recover metal values using thermal plasma coupled with acid leaching -- a response surface modeling approach .
	manualset3
192836	1	415720	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of focal brain ischemia with viral vector-mediated gene transfer .
	manualset3
192837	2	415720	7	NULL	NULL	0	NULL	focal brain ischemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of focal brain ischemia with viral vector-mediated gene transfer .
	manualset3
192838	3	415720	7	NULL	NULL	0	NULL	viral vector-mediated gene transfer	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of focal brain ischemia with viral vector-mediated gene transfer .
	manualset3
192839	1	415721	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of gay men for post-traumatic stress disorder resulting from social ostracism and ridicule : cognitive behavior therapy and eye movement desensitization and reprocessing approaches .
	manualset3
192840	2	415721	7	NULL	NULL	0	NULL	gay men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of gay men for post-traumatic stress disorder resulting from social ostracism and ridicule : cognitive behavior therapy and eye movement desensitization and reprocessing approaches .
	manualset3
192841	3	415721	7	NULL	NULL	0	NULL	post-traumatic stress disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of gay men for post-traumatic stress disorder resulting from social ostracism and ridicule : cognitive behavior therapy and eye movement desensitization and reprocessing approaches .
	manualset3
192842	4	415721	7	NULL	NULL	0	NULL	social ostracism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of gay men for post-traumatic stress disorder resulting from social ostracism and ridicule : cognitive behavior therapy and eye movement desensitization and reprocessing approaches .
	manualset3
192843	5	415721	7	NULL	NULL	0	NULL	ridicule	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of gay men for post-traumatic stress disorder resulting from social ostracism and ridicule : cognitive behavior therapy and eye movement desensitization and reprocessing approaches .
	manualset3
192844	6	415721	7	NULL	NULL	0	NULL	 cognitive behavior therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of gay men for post-traumatic stress disorder resulting from social ostracism and ridicule : cognitive behavior therapy and eye movement desensitization and reprocessing approaches .
	manualset3
192845	7	415721	7	NULL	NULL	NULL	NULL	eye movement desensitization	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Treatment of gay men for post-traumatic stress disorder resulting from social ostracism and ridicule : cognitive behavior therapy and eye movement desensitization and reprocessing approaches .
	manualset3
192846	8	415721	7	NULL	NULL	NULL	NULL	reprocessing approaches	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Treatment of gay men for post-traumatic stress disorder resulting from social ostracism and ridicule : cognitive behavior therapy and eye movement desensitization and reprocessing approaches .
	manualset3
192847	1	415722	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of glial cells with TNF-alpha and IFN-gamma induced only IP-10 , indicating that the expression of chemokine genes other than IP-10 requires a combination of different cytokines or direct cell-cell contact between T cells and glia .
	manualset3
192848	2	415722	7	NULL	NULL	0	NULL	glial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of glial cells with TNF-alpha and IFN-gamma induced only IP-10 , indicating that the expression of chemokine genes other than IP-10 requires a combination of different cytokines or direct cell-cell contact between T cells and glia .
	manualset3
192849	3	415722	7	NULL	NULL	NULL	NULL	IFN-gamma 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Treatment of glial cells with TNF-alpha and IFN-gamma induced only IP-10 , indicating that the expression of chemokine genes other than IP-10 requires a combination of different cytokines or direct cell-cell contact between T cells and glia .
	manualset3
192850	4	415722	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of glial cells with TNF-alpha and IFN-gamma induced only IP-10 , indicating that the expression of chemokine genes other than IP-10 requires a combination of different cytokines or direct cell-cell contact between T cells and glia .
	manualset3
192851	5	415722	7	NULL	NULL	0	NULL	chemokine genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of glial cells with TNF-alpha and IFN-gamma induced only IP-10 , indicating that the expression of chemokine genes other than IP-10 requires a combination of different cytokines or direct cell-cell contact between T cells and glia .
	manualset3
192852	6	415722	7	NULL	NULL	0	NULL	IP-10	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of glial cells with TNF-alpha and IFN-gamma induced only IP-10 , indicating that the expression of chemokine genes other than IP-10 requires a combination of different cytokines or direct cell-cell contact between T cells and glia .
	manualset3
192853	7	415722	7	NULL	NULL	0	NULL	combination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of glial cells with TNF-alpha and IFN-gamma induced only IP-10 , indicating that the expression of chemokine genes other than IP-10 requires a combination of different cytokines or direct cell-cell contact between T cells and glia .
	manualset3
192854	8	415722	7	NULL	NULL	NULL	NULL	 different cytokines 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Treatment of glial cells with TNF-alpha and IFN-gamma induced only IP-10 , indicating that the expression of chemokine genes other than IP-10 requires a combination of different cytokines or direct cell-cell contact between T cells and glia .
	manualset3
192855	9	415722	7	NULL	NULL	0	NULL	direct cell-cell contact	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of glial cells with TNF-alpha and IFN-gamma induced only IP-10 , indicating that the expression of chemokine genes other than IP-10 requires a combination of different cytokines or direct cell-cell contact between T cells and glia .
	manualset3
192856	10	415722	7	NULL	NULL	0	NULL	T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of glial cells with TNF-alpha and IFN-gamma induced only IP-10 , indicating that the expression of chemokine genes other than IP-10 requires a combination of different cytokines or direct cell-cell contact between T cells and glia .
	manualset3
192857	11	415722	7	NULL	NULL	NULL	NULL	glia	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Treatment of glial cells with TNF-alpha and IFN-gamma induced only IP-10 , indicating that the expression of chemokine genes other than IP-10 requires a combination of different cytokines or direct cell-cell contact between T cells and glia .
	manualset3
192858	12	415722	7	NULL	NULL	0	NULL	TNF-alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of glial cells with TNF-alpha and IFN-gamma induced only IP-10 , indicating that the expression of chemokine genes other than IP-10 requires a combination of different cytokines or direct cell-cell contact between T cells and glia .
	manualset3
194210	13	415722	7	NULL	NULL	0	NULL	IP-10	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of glial cells with TNF-alpha and IFN-gamma induced only IP-10 , indicating that the expression of chemokine genes other than IP-10 requires a combination of different cytokines or direct cell-cell contact between T cells and glia .
	manualset3
192859	1	415723	7	NULL	NULL	0	NULL	Treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of hepatic metastases of breast cancer with CT-guided interstitial brachytherapy - a phase II-study .
	manualset3
192860	2	415723	7	NULL	NULL	0	NULL	hepatic metastases	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of hepatic metastases of breast cancer with CT-guided interstitial brachytherapy - a phase II-study .
	manualset3
192861	3	415723	7	NULL	NULL	0	NULL	 breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of hepatic metastases of breast cancer with CT-guided interstitial brachytherapy - a phase II-study .
	manualset3
192862	4	415723	7	NULL	NULL	0	NULL	CT-guided interstitial brachytherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of hepatic metastases of breast cancer with CT-guided interstitial brachytherapy - a phase II-study .
	manualset3
192863	5	415723	7	NULL	NULL	0	NULL	phase II-study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of hepatic metastases of breast cancer with CT-guided interstitial brachytherapy - a phase II-study .
	manualset3
192864	1	415724	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of human macrophages with the PPARalpha ligands bezafibrate or WY14643 inhibited OPN expression .
	manualset3
192865	2	415724	7	NULL	NULL	0	NULL	human macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of human macrophages with the PPARalpha ligands bezafibrate or WY14643 inhibited OPN expression .
	manualset3
192866	3	415724	7	NULL	NULL	0	NULL	PPARalpha ligands bezafibrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of human macrophages with the PPARalpha ligands bezafibrate or WY14643 inhibited OPN expression .
	manualset3
192867	4	415724	7	NULL	NULL	0	NULL	WY14643	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of human macrophages with the PPARalpha ligands bezafibrate or WY14643 inhibited OPN expression .
	manualset3
192868	5	415724	7	NULL	NULL	0	NULL	OPN expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of human macrophages with the PPARalpha ligands bezafibrate or WY14643 inhibited OPN expression .
	manualset3
192869	1	415725	7	NULL	NULL	0	NULL	Treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of patients with high grade non-Hodgkin 's lymphomas and central nervous system involvement : is radiation an essential component of therapy ?
	manualset3
192870	2	415725	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of patients with high grade non-Hodgkin 's lymphomas and central nervous system involvement : is radiation an essential component of therapy ?
	manualset3
192871	3	415725	7	NULL	NULL	0	NULL	high grade non-Hodgkin 's lymphomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of patients with high grade non-Hodgkin 's lymphomas and central nervous system involvement : is radiation an essential component of therapy ?
	manualset3
192872	4	415725	7	NULL	NULL	0	NULL	central nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of patients with high grade non-Hodgkin 's lymphomas and central nervous system involvement : is radiation an essential component of therapy ?
	manualset3
192873	5	415725	7	NULL	NULL	0	NULL	radiation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of patients with high grade non-Hodgkin 's lymphomas and central nervous system involvement : is radiation an essential component of therapy ?
	manualset3
192874	6	415725	7	NULL	NULL	0	NULL	 essential component 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of patients with high grade non-Hodgkin 's lymphomas and central nervous system involvement : is radiation an essential component of therapy ?
	manualset3
192875	7	415725	7	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of patients with high grade non-Hodgkin 's lymphomas and central nervous system involvement : is radiation an essential component of therapy ?
	manualset3
192876	1	415726	7	NULL	NULL	0	NULL	Treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of plasmid DNA with Cr ( III ) ( as CrCl ( 3 ) ) increased DNA binding as a function of dose .
	manualset3
192877	2	415726	7	NULL	NULL	0	NULL	plasmid DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of plasmid DNA with Cr ( III ) ( as CrCl ( 3 ) ) increased DNA binding as a function of dose .
	manualset3
192878	3	415726	7	NULL	NULL	0	NULL	Cr ( III ) ( as CrCl ( 3 ) )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of plasmid DNA with Cr ( III ) ( as CrCl ( 3 ) ) increased DNA binding as a function of dose .
	manualset3
192879	4	415726	7	NULL	NULL	0	NULL	DNA binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of plasmid DNA with Cr ( III ) ( as CrCl ( 3 ) ) increased DNA binding as a function of dose .
	manualset3
192880	5	415726	7	NULL	NULL	0	NULL	 function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of plasmid DNA with Cr ( III ) ( as CrCl ( 3 ) ) increased DNA binding as a function of dose .
	manualset3
192881	6	415726	7	NULL	NULL	0	NULL	 dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of plasmid DNA with Cr ( III ) ( as CrCl ( 3 ) ) increased DNA binding as a function of dose .
	manualset3
192882	1	415727	7	NULL	NULL	0	NULL	 injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After injection of 600 MBq of MIBI , intraoperative nuclear mapping was performed using a hand-held gamma probe .
	manualset3
192883	2	415727	7	NULL	NULL	0	NULL	600 MBq	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After injection of 600 MBq of MIBI , intraoperative nuclear mapping was performed using a hand-held gamma probe .
	manualset3
192884	3	415727	7	NULL	NULL	0	NULL	MIBI	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	After injection of 600 MBq of MIBI , intraoperative nuclear mapping was performed using a hand-held gamma probe .
	manualset3
192885	4	415727	7	NULL	NULL	0	NULL	intraoperative nuclear mapping	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After injection of 600 MBq of MIBI , intraoperative nuclear mapping was performed using a hand-held gamma probe .
	manualset3
192886	5	415727	7	NULL	NULL	0	NULL	hand-held gamma probe	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	After injection of 600 MBq of MIBI , intraoperative nuclear mapping was performed using a hand-held gamma probe .
	manualset3
192887	1	415728	7	NULL	NULL	0	NULL	Treatment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of pulmonary diseases with Chlorocide-aerosol .
	manualset3
192888	2	415728	7	NULL	NULL	0	NULL	 pulmonary diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of pulmonary diseases with Chlorocide-aerosol .
	manualset3
192889	3	415728	7	NULL	NULL	0	NULL	Chlorocide-aerosol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of pulmonary diseases with Chlorocide-aerosol .
	manualset3
192890	1	415729	7	NULL	NULL	0	NULL	Treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of rat and human islets with dsRNA in the form of polyinosinic-polycytidylic acid ( poly IC ) and IFN-gamma resulted in iNOS expression and nitric oxide production .
	manualset3
192891	2	415729	7	NULL	NULL	0	NULL	rat islets	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of rat and human islets with dsRNA in the form of polyinosinic-polycytidylic acid ( poly IC ) and IFN-gamma resulted in iNOS expression and nitric oxide production .
	manualset3
192892	3	415729	7	NULL	NULL	0	NULL	human islets	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of rat and human islets with dsRNA in the form of polyinosinic-polycytidylic acid ( poly IC ) and IFN-gamma resulted in iNOS expression and nitric oxide production .
	manualset3
192893	4	415729	7	NULL	NULL	0	NULL	 dsRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of rat and human islets with dsRNA in the form of polyinosinic-polycytidylic acid ( poly IC ) and IFN-gamma resulted in iNOS expression and nitric oxide production .
	manualset3
192894	5	415729	7	NULL	NULL	0	NULL	polyinosinic-polycytidylic acid ( poly IC )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of rat and human islets with dsRNA in the form of polyinosinic-polycytidylic acid ( poly IC ) and IFN-gamma resulted in iNOS expression and nitric oxide production .
	manualset3
192895	6	415729	7	NULL	NULL	0	NULL	IFN-gamma	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of rat and human islets with dsRNA in the form of polyinosinic-polycytidylic acid ( poly IC ) and IFN-gamma resulted in iNOS expression and nitric oxide production .
	manualset3
192896	7	415729	7	NULL	NULL	0	NULL	iNOS expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of rat and human islets with dsRNA in the form of polyinosinic-polycytidylic acid ( poly IC ) and IFN-gamma resulted in iNOS expression and nitric oxide production .
	manualset3
192897	8	415729	7	NULL	NULL	0	NULL	nitric oxide production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of rat and human islets with dsRNA in the form of polyinosinic-polycytidylic acid ( poly IC ) and IFN-gamma resulted in iNOS expression and nitric oxide production .
	manualset3
192898	1	415730	7	NULL	NULL	0	NULL	Treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of rat reticulocytes with isoproterenol , dibutyryl cAMP and tetradecanoyl phorbol acetate ( TPA ) caused the desensitization of beta-adrenoceptor-coupled adenylate cyclase .
	manualset3
192899	2	415730	7	NULL	NULL	0	NULL	rat reticulocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of rat reticulocytes with isoproterenol , dibutyryl cAMP and tetradecanoyl phorbol acetate ( TPA ) caused the desensitization of beta-adrenoceptor-coupled adenylate cyclase .
	manualset3
192900	3	415730	7	NULL	NULL	0	NULL	isoproterenol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of rat reticulocytes with isoproterenol , dibutyryl cAMP and tetradecanoyl phorbol acetate ( TPA ) caused the desensitization of beta-adrenoceptor-coupled adenylate cyclase .
	manualset3
192901	4	415730	7	NULL	NULL	0	NULL	dibutyryl cAMP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of rat reticulocytes with isoproterenol , dibutyryl cAMP and tetradecanoyl phorbol acetate ( TPA ) caused the desensitization of beta-adrenoceptor-coupled adenylate cyclase .
	manualset3
192902	5	415730	7	NULL	NULL	0	NULL	tetradecanoyl phorbol acetate ( TPA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of rat reticulocytes with isoproterenol , dibutyryl cAMP and tetradecanoyl phorbol acetate ( TPA ) caused the desensitization of beta-adrenoceptor-coupled adenylate cyclase .
	manualset3
192903	6	415730	7	NULL	NULL	0	NULL	desensitization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of rat reticulocytes with isoproterenol , dibutyryl cAMP and tetradecanoyl phorbol acetate ( TPA ) caused the desensitization of beta-adrenoceptor-coupled adenylate cyclase .
	manualset3
192904	7	415730	7	NULL	NULL	0	NULL	beta-adrenoceptor-coupled adenylate cyclase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of rat reticulocytes with isoproterenol , dibutyryl cAMP and tetradecanoyl phorbol acetate ( TPA ) caused the desensitization of beta-adrenoceptor-coupled adenylate cyclase .
	manualset3
193190	1	415731	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of the cells with the specific Jak2 inhibitor tyrphostin AG 490 inhibits myeloid differentiation driven by the distal EpoR .
	manualset3
193191	2	415731	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of the cells with the specific Jak2 inhibitor tyrphostin AG 490 inhibits myeloid differentiation driven by the distal EpoR .
	manualset3
193192	3	415731	7	NULL	NULL	NULL	NULL	specific Jak2 inhibitor tyrphostin AG 490	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Treatment of the cells with the specific Jak2 inhibitor tyrphostin AG 490 inhibits myeloid differentiation driven by the distal EpoR .
	manualset3
193193	4	415731	7	NULL	NULL	0	NULL	myeloid differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of the cells with the specific Jak2 inhibitor tyrphostin AG 490 inhibits myeloid differentiation driven by the distal EpoR .
	manualset3
193194	5	415731	7	NULL	NULL	0	NULL	 distal EpoR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of the cells with the specific Jak2 inhibitor tyrphostin AG 490 inhibits myeloid differentiation driven by the distal EpoR .
	manualset3
193195	1	415732	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of the reduced enzyme with papain followed by acid hydrolysis liberates epsilon-N - ( 3H ) pyridoxyl lysine which is degraded to ( 3H ) pyridoxamine diHCl and stereochemically analyzed with apoaspartate aminotransferase .
	manualset3
193196	2	415732	7	NULL	NULL	0	NULL	reduced enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of the reduced enzyme with papain followed by acid hydrolysis liberates epsilon-N - ( 3H ) pyridoxyl lysine which is degraded to ( 3H ) pyridoxamine diHCl and stereochemically analyzed with apoaspartate aminotransferase .
	manualset3
193197	3	415732	7	NULL	NULL	0	NULL	 papain	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of the reduced enzyme with papain followed by acid hydrolysis liberates epsilon-N - ( 3H ) pyridoxyl lysine which is degraded to ( 3H ) pyridoxamine diHCl and stereochemically analyzed with apoaspartate aminotransferase .
	manualset3
193198	4	415732	7	NULL	NULL	0	NULL	acid hydrolysis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of the reduced enzyme with papain followed by acid hydrolysis liberates epsilon-N - ( 3H ) pyridoxyl lysine which is degraded to ( 3H ) pyridoxamine diHCl and stereochemically analyzed with apoaspartate aminotransferase .
	manualset3
193199	5	415732	7	NULL	NULL	0	NULL	epsilon-N - ( 3H ) pyridoxyl lysine	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of the reduced enzyme with papain followed by acid hydrolysis liberates epsilon-N - ( 3H ) pyridoxyl lysine which is degraded to ( 3H ) pyridoxamine diHCl and stereochemically analyzed with apoaspartate aminotransferase .
	manualset3
193200	6	415732	7	NULL	NULL	0	NULL	( 3H ) pyridoxamine diHCl	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of the reduced enzyme with papain followed by acid hydrolysis liberates epsilon-N - ( 3H ) pyridoxyl lysine which is degraded to ( 3H ) pyridoxamine diHCl and stereochemically analyzed with apoaspartate aminotransferase .
	manualset3
193201	7	415732	7	NULL	NULL	0	NULL	apoaspartate aminotransferase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of the reduced enzyme with papain followed by acid hydrolysis liberates epsilon-N - ( 3H ) pyridoxyl lysine which is degraded to ( 3H ) pyridoxamine diHCl and stereochemically analyzed with apoaspartate aminotransferase .
	manualset3
193202	1	415733	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of urinary tract stones .
	manualset3
193203	2	415733	7	NULL	NULL	0	NULL	urinary tract stones	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of urinary tract stones .
	manualset3
193204	1	415734	7	NULL	NULL	NULL	NULL	 intervention	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After intervention , patients were followed at one , six and 12 month intervals with clinical examination and arterial duplex study .
	manualset3
193205	2	415734	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	After intervention , patients were followed at one , six and 12 month intervals with clinical examination and arterial duplex study .
	manualset3
193206	3	415734	7	NULL	NULL	0	NULL	one month interval	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After intervention , patients were followed at one , six and 12 month intervals with clinical examination and arterial duplex study .
	manualset3
193207	4	415734	7	NULL	NULL	0	NULL	six month interval	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After intervention , patients were followed at one , six and 12 month intervals with clinical examination and arterial duplex study .
	manualset3
193208	5	415734	7	NULL	NULL	0	NULL	12 month intervals	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After intervention , patients were followed at one , six and 12 month intervals with clinical examination and arterial duplex study .
	manualset3
193209	6	415734	7	NULL	NULL	0	NULL	clinical examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After intervention , patients were followed at one , six and 12 month intervals with clinical examination and arterial duplex study .
	manualset3
193210	7	415734	7	NULL	NULL	NULL	NULL	arterial duplex study 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After intervention , patients were followed at one , six and 12 month intervals with clinical examination and arterial duplex study .
	manualset3
193211	1	415735	7	NULL	NULL	NULL	NULL	Treatment persistency	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Treatment persistency was defined as the absence of a & gt ; 45 day gap between ZOL administrations .
	manualset3
193212	2	415735	7	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment persistency was defined as the absence of a & gt ; 45 day gap between ZOL administrations .
	manualset3
193213	3	415735	7	NULL	NULL	0	NULL	a & gt	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment persistency was defined as the absence of a & gt ; 45 day gap between ZOL administrations .
	manualset3
193214	4	415735	7	NULL	NULL	0	NULL	45 day gap	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment persistency was defined as the absence of a & gt ; 45 day gap between ZOL administrations .
	manualset3
193215	5	415735	7	NULL	NULL	0	NULL	ZOL administrations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment persistency was defined as the absence of a & gt ; 45 day gap between ZOL administrations .
	manualset3
193216	1	415736	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment resulted in a reduction of tonsillar size with minimal pain , which can be attributed to the avoidance of mucosal interruption .
	manualset3
193217	2	415736	7	NULL	NULL	0	NULL	reduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment resulted in a reduction of tonsillar size with minimal pain , which can be attributed to the avoidance of mucosal interruption .
	manualset3
193218	3	415736	7	NULL	NULL	0	NULL	tonsillar size	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment resulted in a reduction of tonsillar size with minimal pain , which can be attributed to the avoidance of mucosal interruption .
	manualset3
193219	4	415736	7	NULL	NULL	0	NULL	minimal pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment resulted in a reduction of tonsillar size with minimal pain , which can be attributed to the avoidance of mucosal interruption .
	manualset3
193220	5	415736	7	NULL	NULL	0	NULL	avoidance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment resulted in a reduction of tonsillar size with minimal pain , which can be attributed to the avoidance of mucosal interruption .
	manualset3
193221	6	415736	7	NULL	NULL	0	NULL	mucosal interruption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment resulted in a reduction of tonsillar size with minimal pain , which can be attributed to the avoidance of mucosal interruption .
	manualset3
193228	1	415737	7	NULL	NULL	0	NULL	Treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment revolves around supportive care and prevention of complications .
	manualset3
193238	2	415737	7	NULL	NULL	0	NULL	supportive care	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment revolves around supportive care and prevention of complications .
	manualset3
193239	3	415737	7	NULL	NULL	0	NULL	prevention 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment revolves around supportive care and prevention of complications .
	manualset3
193240	4	415737	7	NULL	NULL	0	NULL	complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment revolves around supportive care and prevention of complications .
	manualset3
193241	1	415738	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment was attempted with the Sampson pericortical bone clamp , but was unsuccessful .
	manualset3
193242	2	415738	7	NULL	NULL	0	NULL	Sampson pericortical bone clamp	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment was attempted with the Sampson pericortical bone clamp , but was unsuccessful .
	manualset3
193243	1	415739	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment was with 3 x 10 ( -7 ) M NPY or 10 ( -7 ) g/ml VEGF for 2 h along with specific inhibitors .
	manualset3
193244	2	415739	7	NULL	NULL	0	NULL	 3 x 10 ( -7 ) M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment was with 3 x 10 ( -7 ) M NPY or 10 ( -7 ) g/ml VEGF for 2 h along with specific inhibitors .
	manualset3
193245	3	415739	7	NULL	NULL	0	NULL	NPY	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment was with 3 x 10 ( -7 ) M NPY or 10 ( -7 ) g/ml VEGF for 2 h along with specific inhibitors .
	manualset3
193246	4	415739	7	NULL	NULL	0	NULL	10 ( -7 ) g/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment was with 3 x 10 ( -7 ) M NPY or 10 ( -7 ) g/ml VEGF for 2 h along with specific inhibitors .
	manualset3
193247	5	415739	7	NULL	NULL	0	NULL	VEGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment was with 3 x 10 ( -7 ) M NPY or 10 ( -7 ) g/ml VEGF for 2 h along with specific inhibitors .
	manualset3
193248	6	415739	7	NULL	NULL	0	NULL	2 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment was with 3 x 10 ( -7 ) M NPY or 10 ( -7 ) g/ml VEGF for 2 h along with specific inhibitors .
	manualset3
193249	7	415739	7	NULL	NULL	0	NULL	specific inhibitors 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment was with 3 x 10 ( -7 ) M NPY or 10 ( -7 ) g/ml VEGF for 2 h along with specific inhibitors .
	manualset3
193254	1	415740	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with 1 g/kg 3-AT attenuated HS-mediated cardioprotection ( 36.9 + / - 4.9 % , P = 0.063 vs. HS ) ; protection was abolished with 2 g/kg 3-AT ( 48.9 + / - 6.6 % ) .
	manualset3
193255	2	415740	7	NULL	NULL	0	NULL	1 g/kg 3-AT	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with 1 g/kg 3-AT attenuated HS-mediated cardioprotection ( 36.9 + / - 4.9 % , P = 0.063 vs. HS ) ; protection was abolished with 2 g/kg 3-AT ( 48.9 + / - 6.6 % ) .
	manualset3
193257	3	415740	7	NULL	NULL	0	NULL	HS-mediated cardioprotection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with 1 g/kg 3-AT attenuated HS-mediated cardioprotection ( 36.9 + / - 4.9 % , P = 0.063 vs. HS ) ; protection was abolished with 2 g/kg 3-AT ( 48.9 + / - 6.6 % ) .
	manualset3
193258	4	415740	7	NULL	NULL	0	NULL	36.9 + / - 4.9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with 1 g/kg 3-AT attenuated HS-mediated cardioprotection ( 36.9 + / - 4.9 % , P = 0.063 vs. HS ) ; protection was abolished with 2 g/kg 3-AT ( 48.9 + / - 6.6 % ) .
	manualset3
193259	5	415740	7	NULL	NULL	0	NULL	P = 0.063 vs. HS	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with 1 g/kg 3-AT attenuated HS-mediated cardioprotection ( 36.9 + / - 4.9 % , P = 0.063 vs. HS ) ; protection was abolished with 2 g/kg 3-AT ( 48.9 + / - 6.6 % ) .
	manualset3
193260	6	415740	7	NULL	NULL	0	NULL	protection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with 1 g/kg 3-AT attenuated HS-mediated cardioprotection ( 36.9 + / - 4.9 % , P = 0.063 vs. HS ) ; protection was abolished with 2 g/kg 3-AT ( 48.9 + / - 6.6 % ) .
	manualset3
193261	7	415740	7	NULL	NULL	0	NULL	2 g/kg 3-AT	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with 1 g/kg 3-AT attenuated HS-mediated cardioprotection ( 36.9 + / - 4.9 % , P = 0.063 vs. HS ) ; protection was abolished with 2 g/kg 3-AT ( 48.9 + / - 6.6 % ) .
	manualset3
193262	8	415740	7	NULL	NULL	0	NULL	48.9 + / - 6.6 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with 1 g/kg 3-AT attenuated HS-mediated cardioprotection ( 36.9 + / - 4.9 % , P = 0.063 vs. HS ) ; protection was abolished with 2 g/kg 3-AT ( 48.9 + / - 6.6 % ) .
	manualset3
193267	1	415741	7	NULL	NULL	NULL	NULL	intravenous inoculation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After intravenous inoculation of guinea pigs , the initial ratio of bacteria in maternal organs to placenta was 10 ( 3 ) -10 ( 4 ) : 1 .
	manualset3
193270	2	415741	7	NULL	NULL	0	NULL	guinea pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	After intravenous inoculation of guinea pigs , the initial ratio of bacteria in maternal organs to placenta was 10 ( 3 ) -10 ( 4 ) : 1 .
	manualset3
193272	3	415741	7	NULL	NULL	0	NULL	initial ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After intravenous inoculation of guinea pigs , the initial ratio of bacteria in maternal organs to placenta was 10 ( 3 ) -10 ( 4 ) : 1 .
	manualset3
193274	4	415741	7	NULL	NULL	0	NULL	bacteria 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	After intravenous inoculation of guinea pigs , the initial ratio of bacteria in maternal organs to placenta was 10 ( 3 ) -10 ( 4 ) : 1 .
	manualset3
193276	5	415741	7	NULL	NULL	0	NULL	maternal organs 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After intravenous inoculation of guinea pigs , the initial ratio of bacteria in maternal organs to placenta was 10 ( 3 ) -10 ( 4 ) : 1 .
	manualset3
193277	6	415741	7	NULL	NULL	0	NULL	placenta	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After intravenous inoculation of guinea pigs , the initial ratio of bacteria in maternal organs to placenta was 10 ( 3 ) -10 ( 4 ) : 1 .
	manualset3
193278	7	415741	7	NULL	NULL	0	NULL	10 ( 3 ) -10 ( 4 ) : 1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	After intravenous inoculation of guinea pigs , the initial ratio of bacteria in maternal organs to placenta was 10 ( 3 ) -10 ( 4 ) : 1 .
	manualset3
193284	1	415742	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with 5-hydroxytryptophan ( 20 mg/kg ) increased the concentration of 5-HT in the brain of rats pretreated with either NaCl or PCPA and enhanced the inhibitory effect of CCK-8 on ingestive behavior in the PCPA - , but not NaCl - , treated rats .
	manualset3
193285	2	415742	7	NULL	NULL	0	NULL	5-hydroxytryptophan ( 20 mg/kg )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with 5-hydroxytryptophan ( 20 mg/kg ) increased the concentration of 5-HT in the brain of rats pretreated with either NaCl or PCPA and enhanced the inhibitory effect of CCK-8 on ingestive behavior in the PCPA - , but not NaCl - , treated rats .
	manualset3
193286	3	415742	7	NULL	NULL	0	NULL	concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with 5-hydroxytryptophan ( 20 mg/kg ) increased the concentration of 5-HT in the brain of rats pretreated with either NaCl or PCPA and enhanced the inhibitory effect of CCK-8 on ingestive behavior in the PCPA - , but not NaCl - , treated rats .
	manualset3
193287	4	415742	7	NULL	NULL	0	NULL	5-HT	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with 5-hydroxytryptophan ( 20 mg/kg ) increased the concentration of 5-HT in the brain of rats pretreated with either NaCl or PCPA and enhanced the inhibitory effect of CCK-8 on ingestive behavior in the PCPA - , but not NaCl - , treated rats .
	manualset3
193288	5	415742	7	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with 5-hydroxytryptophan ( 20 mg/kg ) increased the concentration of 5-HT in the brain of rats pretreated with either NaCl or PCPA and enhanced the inhibitory effect of CCK-8 on ingestive behavior in the PCPA - , but not NaCl - , treated rats .
	manualset3
193289	6	415742	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with 5-hydroxytryptophan ( 20 mg/kg ) increased the concentration of 5-HT in the brain of rats pretreated with either NaCl or PCPA and enhanced the inhibitory effect of CCK-8 on ingestive behavior in the PCPA - , but not NaCl - , treated rats .
	manualset3
193291	7	415742	7	NULL	NULL	0	NULL	NaCl 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with 5-hydroxytryptophan ( 20 mg/kg ) increased the concentration of 5-HT in the brain of rats pretreated with either NaCl or PCPA and enhanced the inhibitory effect of CCK-8 on ingestive behavior in the PCPA - , but not NaCl - , treated rats .
	manualset3
193292	8	415742	7	NULL	NULL	0	NULL	PCPA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with 5-hydroxytryptophan ( 20 mg/kg ) increased the concentration of 5-HT in the brain of rats pretreated with either NaCl or PCPA and enhanced the inhibitory effect of CCK-8 on ingestive behavior in the PCPA - , but not NaCl - , treated rats .
	manualset3
193296	9	415742	7	NULL	NULL	0	NULL	inhibitory effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with 5-hydroxytryptophan ( 20 mg/kg ) increased the concentration of 5-HT in the brain of rats pretreated with either NaCl or PCPA and enhanced the inhibitory effect of CCK-8 on ingestive behavior in the PCPA - , but not NaCl - , treated rats .
	manualset3
193299	10	415742	7	NULL	NULL	0	NULL	CCK-8	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with 5-hydroxytryptophan ( 20 mg/kg ) increased the concentration of 5-HT in the brain of rats pretreated with either NaCl or PCPA and enhanced the inhibitory effect of CCK-8 on ingestive behavior in the PCPA - , but not NaCl - , treated rats .
	manualset3
193301	11	415742	7	NULL	NULL	0	NULL	ingestive behavior	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with 5-hydroxytryptophan ( 20 mg/kg ) increased the concentration of 5-HT in the brain of rats pretreated with either NaCl or PCPA and enhanced the inhibitory effect of CCK-8 on ingestive behavior in the PCPA - , but not NaCl - , treated rats .
	manualset3
193302	12	415742	7	NULL	NULL	0	NULL	PCPA - treated rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with 5-hydroxytryptophan ( 20 mg/kg ) increased the concentration of 5-HT in the brain of rats pretreated with either NaCl or PCPA and enhanced the inhibitory effect of CCK-8 on ingestive behavior in the PCPA - , but not NaCl - , treated rats .
	manualset3
193303	13	415742	7	NULL	NULL	0	NULL	NaCl - , treated rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with 5-hydroxytryptophan ( 20 mg/kg ) increased the concentration of 5-HT in the brain of rats pretreated with either NaCl or PCPA and enhanced the inhibitory effect of CCK-8 on ingestive behavior in the PCPA - , but not NaCl - , treated rats .
	manualset3
193310	1	415743	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with 5 mM dithiothreitol significantly ( P & lt ; 0.01 ) reduced the angiotensin II-induced contractile response to 1.2 % in the rabbit aorta , but it did not significantly reduce the response in the canine aorta ( 83.2 % ) .
	manualset3
193313	2	415743	7	NULL	NULL	0	NULL	5 mM dithiothreitol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with 5 mM dithiothreitol significantly ( P & lt ; 0.01 ) reduced the angiotensin II-induced contractile response to 1.2 % in the rabbit aorta , but it did not significantly reduce the response in the canine aorta ( 83.2 % ) .
	manualset3
193314	3	415743	7	NULL	NULL	0	NULL	 P & lt ; 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with 5 mM dithiothreitol significantly ( P & lt ; 0.01 ) reduced the angiotensin II-induced contractile response to 1.2 % in the rabbit aorta , but it did not significantly reduce the response in the canine aorta ( 83.2 % ) .
	manualset3
193315	4	415743	7	NULL	NULL	0	NULL	angiotensin II-induced contractile response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with 5 mM dithiothreitol significantly ( P & lt ; 0.01 ) reduced the angiotensin II-induced contractile response to 1.2 % in the rabbit aorta , but it did not significantly reduce the response in the canine aorta ( 83.2 % ) .
	manualset3
193317	5	415743	7	NULL	NULL	0	NULL	1.2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with 5 mM dithiothreitol significantly ( P & lt ; 0.01 ) reduced the angiotensin II-induced contractile response to 1.2 % in the rabbit aorta , but it did not significantly reduce the response in the canine aorta ( 83.2 % ) .
	manualset3
193319	6	415743	7	NULL	NULL	0	NULL	rabbit aorta	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with 5 mM dithiothreitol significantly ( P & lt ; 0.01 ) reduced the angiotensin II-induced contractile response to 1.2 % in the rabbit aorta , but it did not significantly reduce the response in the canine aorta ( 83.2 % ) .
	manualset3
193321	7	415743	7	NULL	NULL	0	NULL	response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with 5 mM dithiothreitol significantly ( P & lt ; 0.01 ) reduced the angiotensin II-induced contractile response to 1.2 % in the rabbit aorta , but it did not significantly reduce the response in the canine aorta ( 83.2 % ) .
	manualset3
193323	8	415743	7	NULL	NULL	0	NULL	canine aorta	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with 5 mM dithiothreitol significantly ( P & lt ; 0.01 ) reduced the angiotensin II-induced contractile response to 1.2 % in the rabbit aorta , but it did not significantly reduce the response in the canine aorta ( 83.2 % ) .
	manualset3
193324	9	415743	7	NULL	NULL	0	NULL	83.2 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with 5 mM dithiothreitol significantly ( P & lt ; 0.01 ) reduced the angiotensin II-induced contractile response to 1.2 % in the rabbit aorta , but it did not significantly reduce the response in the canine aorta ( 83.2 % ) .
	manualset3
193330	1	415744	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with AMB-NIV resulted in significantly higher drug levels in the lungs and skin ( p & lt ; 0.05 ) compared to similar treatment with AMB solution but significantly lower plasma levels ( p & lt ; 0.05 ) .
	manualset3
193335	2	415744	7	NULL	NULL	0	NULL	AMB-NIV	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with AMB-NIV resulted in significantly higher drug levels in the lungs and skin ( p & lt ; 0.05 ) compared to similar treatment with AMB solution but significantly lower plasma levels ( p & lt ; 0.05 ) .
	manualset3
193336	3	415744	7	NULL	NULL	0	NULL	drug levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with AMB-NIV resulted in significantly higher drug levels in the lungs and skin ( p & lt ; 0.05 ) compared to similar treatment with AMB solution but significantly lower plasma levels ( p & lt ; 0.05 ) .
	manualset3
193337	4	415744	7	NULL	NULL	0	NULL	 lungs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with AMB-NIV resulted in significantly higher drug levels in the lungs and skin ( p & lt ; 0.05 ) compared to similar treatment with AMB solution but significantly lower plasma levels ( p & lt ; 0.05 ) .
	manualset3
193338	5	415744	7	NULL	NULL	0	NULL	skin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with AMB-NIV resulted in significantly higher drug levels in the lungs and skin ( p & lt ; 0.05 ) compared to similar treatment with AMB solution but significantly lower plasma levels ( p & lt ; 0.05 ) .
	manualset3
193339	6	415744	7	NULL	NULL	0	NULL	p & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with AMB-NIV resulted in significantly higher drug levels in the lungs and skin ( p & lt ; 0.05 ) compared to similar treatment with AMB solution but significantly lower plasma levels ( p & lt ; 0.05 ) .
	manualset3
193340	7	415744	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with AMB-NIV resulted in significantly higher drug levels in the lungs and skin ( p & lt ; 0.05 ) compared to similar treatment with AMB solution but significantly lower plasma levels ( p & lt ; 0.05 ) .
	manualset3
193341	8	415744	7	NULL	NULL	0	NULL	AMB solution	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with AMB-NIV resulted in significantly higher drug levels in the lungs and skin ( p & lt ; 0.05 ) compared to similar treatment with AMB solution but significantly lower plasma levels ( p & lt ; 0.05 ) .
	manualset3
193343	9	415744	7	NULL	NULL	0	NULL	lower plasma levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with AMB-NIV resulted in significantly higher drug levels in the lungs and skin ( p & lt ; 0.05 ) compared to similar treatment with AMB solution but significantly lower plasma levels ( p & lt ; 0.05 ) .
	manualset3
193346	10	415744	7	NULL	NULL	0	NULL	p & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with AMB-NIV resulted in significantly higher drug levels in the lungs and skin ( p & lt ; 0.05 ) compared to similar treatment with AMB solution but significantly lower plasma levels ( p & lt ; 0.05 ) .
	manualset3
193348	1	415745	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with DNA-like chimeric molecules inhibited B - and T-cell proliferation , restricted the number of anti-DNA antibody-producing cells and suppressed the generation of IgG anti-DNA antibodies .
	manualset3
193350	2	415745	7	NULL	NULL	0	NULL	DNA-like chimeric molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with DNA-like chimeric molecules inhibited B - and T-cell proliferation , restricted the number of anti-DNA antibody-producing cells and suppressed the generation of IgG anti-DNA antibodies .
	manualset3
193351	3	415745	7	NULL	NULL	NULL	NULL	B-cell proliferation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Treatment with DNA-like chimeric molecules inhibited B - and T-cell proliferation , restricted the number of anti-DNA antibody-producing cells and suppressed the generation of IgG anti-DNA antibodies .
	manualset3
193352	4	415745	7	NULL	NULL	NULL	NULL	T-cell proliferation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Treatment with DNA-like chimeric molecules inhibited B - and T-cell proliferation , restricted the number of anti-DNA antibody-producing cells and suppressed the generation of IgG anti-DNA antibodies .
	manualset3
193354	5	415745	7	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with DNA-like chimeric molecules inhibited B - and T-cell proliferation , restricted the number of anti-DNA antibody-producing cells and suppressed the generation of IgG anti-DNA antibodies .
	manualset3
193355	6	415745	7	NULL	NULL	0	NULL	anti-DNA antibody-producing cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with DNA-like chimeric molecules inhibited B - and T-cell proliferation , restricted the number of anti-DNA antibody-producing cells and suppressed the generation of IgG anti-DNA antibodies .
	manualset3
193356	7	415745	7	NULL	NULL	0	NULL	generation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with DNA-like chimeric molecules inhibited B - and T-cell proliferation , restricted the number of anti-DNA antibody-producing cells and suppressed the generation of IgG anti-DNA antibodies .
	manualset3
193357	8	415745	7	NULL	NULL	0	NULL	IgG anti-DNA antibodies 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with DNA-like chimeric molecules inhibited B - and T-cell proliferation , restricted the number of anti-DNA antibody-producing cells and suppressed the generation of IgG anti-DNA antibodies .
	manualset3
193417	1	415746	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with GDNF promoted the development of two-cell-stage embryos into blastocysts showing increased cell proliferation and decreased apoptosis mainly in trophectoderm cells .
	manualset3
193434	2	415746	7	NULL	NULL	0	NULL	GDNF	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with GDNF promoted the development of two-cell-stage embryos into blastocysts showing increased cell proliferation and decreased apoptosis mainly in trophectoderm cells .
	manualset3
193435	3	415746	7	NULL	NULL	0	NULL	development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with GDNF promoted the development of two-cell-stage embryos into blastocysts showing increased cell proliferation and decreased apoptosis mainly in trophectoderm cells .
	manualset3
193436	4	415746	7	NULL	NULL	0	NULL	two-cell-stage embryos	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with GDNF promoted the development of two-cell-stage embryos into blastocysts showing increased cell proliferation and decreased apoptosis mainly in trophectoderm cells .
	manualset3
193437	5	415746	7	NULL	NULL	0	NULL	blastocysts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with GDNF promoted the development of two-cell-stage embryos into blastocysts showing increased cell proliferation and decreased apoptosis mainly in trophectoderm cells .
	manualset3
193438	6	415746	7	NULL	NULL	0	NULL	increased cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with GDNF promoted the development of two-cell-stage embryos into blastocysts showing increased cell proliferation and decreased apoptosis mainly in trophectoderm cells .
	manualset3
193439	7	415746	7	NULL	NULL	0	NULL	decreased apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with GDNF promoted the development of two-cell-stage embryos into blastocysts showing increased cell proliferation and decreased apoptosis mainly in trophectoderm cells .
	manualset3
193440	8	415746	7	NULL	NULL	0	NULL	trophectoderm cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with GDNF promoted the development of two-cell-stage embryos into blastocysts showing increased cell proliferation and decreased apoptosis mainly in trophectoderm cells .
	manualset3
193441	1	415747	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with GGsTop ( 1 and 10 mg/kg i.v. ) 5 min before ischemia attenuated the ischemia/reperfusion-induced renal dysfunction in a dose-dependent manner .
	manualset3
193442	2	415747	7	NULL	NULL	0	NULL	GGsTop	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with GGsTop ( 1 and 10 mg/kg i.v. ) 5 min before ischemia attenuated the ischemia/reperfusion-induced renal dysfunction in a dose-dependent manner .
	manualset3
193443	3	415747	7	NULL	NULL	0	NULL	1 and 10 mg/kg i.v.	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with GGsTop ( 1 and 10 mg/kg i.v. ) 5 min before ischemia attenuated the ischemia/reperfusion-induced renal dysfunction in a dose-dependent manner .
	manualset3
193444	4	415747	7	NULL	NULL	0	NULL	5 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with GGsTop ( 1 and 10 mg/kg i.v. ) 5 min before ischemia attenuated the ischemia/reperfusion-induced renal dysfunction in a dose-dependent manner .
	manualset3
193445	5	415747	7	NULL	NULL	0	NULL	 ischemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with GGsTop ( 1 and 10 mg/kg i.v. ) 5 min before ischemia attenuated the ischemia/reperfusion-induced renal dysfunction in a dose-dependent manner .
	manualset3
193446	6	415747	7	NULL	NULL	NULL	NULL	ischemia/reperfusion-induced renal dysfunction	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Treatment with GGsTop ( 1 and 10 mg/kg i.v. ) 5 min before ischemia attenuated the ischemia/reperfusion-induced renal dysfunction in a dose-dependent manner .
	manualset3
193447	7	415747	7	NULL	NULL	0	NULL	dose-dependent manner	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with GGsTop ( 1 and 10 mg/kg i.v. ) 5 min before ischemia attenuated the ischemia/reperfusion-induced renal dysfunction in a dose-dependent manner .
	manualset3
193448	1	415748	7	NULL	NULL	0	NULL	Treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with IFN-alpha2b was associated with a 4.8-fold increase in the endogenous production of IL-1Ra in cultured blood sustained over 24 hs .
	manualset3
193449	2	415748	7	NULL	NULL	0	NULL	IFN-alpha2b	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with IFN-alpha2b was associated with a 4.8-fold increase in the endogenous production of IL-1Ra in cultured blood sustained over 24 hs .
	manualset3
193450	3	415748	7	NULL	NULL	0	NULL	 4.8-fold increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with IFN-alpha2b was associated with a 4.8-fold increase in the endogenous production of IL-1Ra in cultured blood sustained over 24 hs .
	manualset3
193451	4	415748	7	NULL	NULL	0	NULL	endogenous production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with IFN-alpha2b was associated with a 4.8-fold increase in the endogenous production of IL-1Ra in cultured blood sustained over 24 hs .
	manualset3
193452	5	415748	7	NULL	NULL	0	NULL	IL-1Ra	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with IFN-alpha2b was associated with a 4.8-fold increase in the endogenous production of IL-1Ra in cultured blood sustained over 24 hs .
	manualset3
193453	6	415748	7	NULL	NULL	0	NULL	cultured blood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with IFN-alpha2b was associated with a 4.8-fold increase in the endogenous production of IL-1Ra in cultured blood sustained over 24 hs .
	manualset3
193454	7	415748	7	NULL	NULL	0	NULL	24 hs	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with IFN-alpha2b was associated with a 4.8-fold increase in the endogenous production of IL-1Ra in cultured blood sustained over 24 hs .
	manualset3
193455	1	415749	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with LMWH initiated at 6 h after thrombin injection only partially ameliorated brain damage .
	manualset3
193456	2	415749	7	NULL	NULL	0	NULL	LMWH	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with LMWH initiated at 6 h after thrombin injection only partially ameliorated brain damage .
	manualset3
193457	3	415749	7	NULL	NULL	0	NULL	6 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with LMWH initiated at 6 h after thrombin injection only partially ameliorated brain damage .
	manualset3
193458	4	415749	7	NULL	NULL	0	NULL	thrombin injection 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with LMWH initiated at 6 h after thrombin injection only partially ameliorated brain damage .
	manualset3
193459	5	415749	7	NULL	NULL	0	NULL	ameliorated brain damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with LMWH initiated at 6 h after thrombin injection only partially ameliorated brain damage .
	manualset3
193460	1	415750	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with Met-RANTES had no effect on the viral titers .
	manualset3
193461	2	415750	7	NULL	NULL	0	NULL	Met-RANTES	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with Met-RANTES had no effect on the viral titers .
	manualset3
193462	3	415750	7	NULL	NULL	0	NULL	 viral titers	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with Met-RANTES had no effect on the viral titers .
	manualset3
193463	1	415751	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with Met increased these levels significantly , with a similar effect on GSH levels in non-diabetic rats .
	manualset3
193464	2	415751	7	NULL	NULL	0	NULL	Met	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with Met increased these levels significantly , with a similar effect on GSH levels in non-diabetic rats .
	manualset3
193465	3	415751	7	NULL	NULL	0	NULL	 levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with Met increased these levels significantly , with a similar effect on GSH levels in non-diabetic rats .
	manualset3
193466	4	415751	7	NULL	NULL	0	NULL	GSH levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with Met increased these levels significantly , with a similar effect on GSH levels in non-diabetic rats .
	manualset3
193467	5	415751	7	NULL	NULL	0	NULL	 non-diabetic rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with Met increased these levels significantly , with a similar effect on GSH levels in non-diabetic rats .
	manualset3
195579	6	415751	7	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with Met increased these levels significantly , with a similar effect on GSH levels in non-diabetic rats .
	manualset3
193468	1	415752	7	NULL	NULL	0	NULL	Condition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Condition of the lymphatic system in 867 cases of cancer of the tongue and breast ) .
	manualset3
193469	2	415752	7	NULL	NULL	0	NULL	lymphatic system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Condition of the lymphatic system in 867 cases of cancer of the tongue and breast ) .
	manualset3
193470	3	415752	7	NULL	NULL	0	NULL	867 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Condition of the lymphatic system in 867 cases of cancer of the tongue and breast ) .
	manualset3
193471	4	415752	7	NULL	NULL	0	NULL	cancer of the tongue	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Condition of the lymphatic system in 867 cases of cancer of the tongue and breast ) .
	manualset3
193472	5	415752	7	NULL	NULL	0	NULL	cancer of the breast	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Condition of the lymphatic system in 867 cases of cancer of the tongue and breast ) .
	manualset3
193473	1	415753	7	NULL	NULL	0	NULL	Treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with NAC had no effect on lung or liver glutathione ( reduced ) ( GSH ) concentrations either after 2 hr post-administration , or over the full 72 hr experimental period .
	manualset3
193474	2	415753	7	NULL	NULL	0	NULL	NAC	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with NAC had no effect on lung or liver glutathione ( reduced ) ( GSH ) concentrations either after 2 hr post-administration , or over the full 72 hr experimental period .
	manualset3
193475	3	415753	7	NULL	NULL	0	NULL	no effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with NAC had no effect on lung or liver glutathione ( reduced ) ( GSH ) concentrations either after 2 hr post-administration , or over the full 72 hr experimental period .
	manualset3
193476	4	415753	7	NULL	NULL	0	NULL	 lung	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with NAC had no effect on lung or liver glutathione ( reduced ) ( GSH ) concentrations either after 2 hr post-administration , or over the full 72 hr experimental period .
	manualset3
193477	5	415753	7	NULL	NULL	0	NULL	 liver glutathione ( reduced ) ( GSH ) concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with NAC had no effect on lung or liver glutathione ( reduced ) ( GSH ) concentrations either after 2 hr post-administration , or over the full 72 hr experimental period .
	manualset3
193478	6	415753	7	NULL	NULL	0	NULL	2 hr post-administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with NAC had no effect on lung or liver glutathione ( reduced ) ( GSH ) concentrations either after 2 hr post-administration , or over the full 72 hr experimental period .
	manualset3
193479	7	415753	7	NULL	NULL	0	NULL	full 72 hr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with NAC had no effect on lung or liver glutathione ( reduced ) ( GSH ) concentrations either after 2 hr post-administration , or over the full 72 hr experimental period .
	manualset3
193480	8	415753	7	NULL	NULL	0	NULL	experimental period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with NAC had no effect on lung or liver glutathione ( reduced ) ( GSH ) concentrations either after 2 hr post-administration , or over the full 72 hr experimental period .
	manualset3
193481	1	415754	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with PPT or DPN did not augment anti-DNP antibody production after DNP-KLH immunization as E ( 2 ) did , implying that not merely one ER signaling pathway is involved in mediating estrogen 's effects on specific humoral immune responses .
	manualset3
193482	2	415754	7	NULL	NULL	0	NULL	PPT	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with PPT or DPN did not augment anti-DNP antibody production after DNP-KLH immunization as E ( 2 ) did , implying that not merely one ER signaling pathway is involved in mediating estrogen 's effects on specific humoral immune responses .
	manualset3
193483	3	415754	7	NULL	NULL	0	NULL	DPN	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with PPT or DPN did not augment anti-DNP antibody production after DNP-KLH immunization as E ( 2 ) did , implying that not merely one ER signaling pathway is involved in mediating estrogen 's effects on specific humoral immune responses .
	manualset3
193484	4	415754	7	NULL	NULL	0	NULL	anti-DNP antibody production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with PPT or DPN did not augment anti-DNP antibody production after DNP-KLH immunization as E ( 2 ) did , implying that not merely one ER signaling pathway is involved in mediating estrogen 's effects on specific humoral immune responses .
	manualset3
193485	5	415754	7	NULL	NULL	0	NULL	DNP-KLH immunization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with PPT or DPN did not augment anti-DNP antibody production after DNP-KLH immunization as E ( 2 ) did , implying that not merely one ER signaling pathway is involved in mediating estrogen 's effects on specific humoral immune responses .
	manualset3
193486	6	415754	7	NULL	NULL	0	NULL	E ( 2 ) 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with PPT or DPN did not augment anti-DNP antibody production after DNP-KLH immunization as E ( 2 ) did , implying that not merely one ER signaling pathway is involved in mediating estrogen 's effects on specific humoral immune responses .
	manualset3
193487	7	415754	7	NULL	NULL	NULL	NULL	one ER signaling pathway 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Treatment with PPT or DPN did not augment anti-DNP antibody production after DNP-KLH immunization as E ( 2 ) did , implying that not merely one ER signaling pathway is involved in mediating estrogen 's effects on specific humoral immune responses .
	manualset3
193488	8	415754	7	NULL	NULL	0	NULL	estrogen 's effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with PPT or DPN did not augment anti-DNP antibody production after DNP-KLH immunization as E ( 2 ) did , implying that not merely one ER signaling pathway is involved in mediating estrogen 's effects on specific humoral immune responses .
	manualset3
193489	9	415754	7	NULL	NULL	0	NULL	specific humoral immune responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with PPT or DPN did not augment anti-DNP antibody production after DNP-KLH immunization as E ( 2 ) did , implying that not merely one ER signaling pathway is involved in mediating estrogen 's effects on specific humoral immune responses .
	manualset3
193490	1	415755	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with caffeine similarly activated CYP1A2 and related monooxygenases as well as UGT , while treatment with catechins induced UGT activity but not 7-ECOD or CN1D activity .
	manualset3
193491	2	415755	7	NULL	NULL	0	NULL	caffeine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with caffeine similarly activated CYP1A2 and related monooxygenases as well as UGT , while treatment with catechins induced UGT activity but not 7-ECOD or CN1D activity .
	manualset3
193492	3	415755	7	NULL	NULL	0	NULL	activated CYP1A2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with caffeine similarly activated CYP1A2 and related monooxygenases as well as UGT , while treatment with catechins induced UGT activity but not 7-ECOD or CN1D activity .
	manualset3
193493	4	415755	7	NULL	NULL	0	NULL	monooxygenases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with caffeine similarly activated CYP1A2 and related monooxygenases as well as UGT , while treatment with catechins induced UGT activity but not 7-ECOD or CN1D activity .
	manualset3
193494	5	415755	7	NULL	NULL	0	NULL	UGT	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with caffeine similarly activated CYP1A2 and related monooxygenases as well as UGT , while treatment with catechins induced UGT activity but not 7-ECOD or CN1D activity .
	manualset3
193495	6	415755	7	NULL	NULL	0	NULL	 treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with caffeine similarly activated CYP1A2 and related monooxygenases as well as UGT , while treatment with catechins induced UGT activity but not 7-ECOD or CN1D activity .
	manualset3
193496	7	415755	7	NULL	NULL	0	NULL	catechins	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with caffeine similarly activated CYP1A2 and related monooxygenases as well as UGT , while treatment with catechins induced UGT activity but not 7-ECOD or CN1D activity .
	manualset3
193497	8	415755	7	NULL	NULL	0	NULL	UGT activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with caffeine similarly activated CYP1A2 and related monooxygenases as well as UGT , while treatment with catechins induced UGT activity but not 7-ECOD or CN1D activity .
	manualset3
193498	9	415755	7	NULL	NULL	0	NULL	7-ECOD activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with caffeine similarly activated CYP1A2 and related monooxygenases as well as UGT , while treatment with catechins induced UGT activity but not 7-ECOD or CN1D activity .
	manualset3
193499	10	415755	7	NULL	NULL	0	NULL	CN1D activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with caffeine similarly activated CYP1A2 and related monooxygenases as well as UGT , while treatment with catechins induced UGT activity but not 7-ECOD or CN1D activity .
	manualset3
193500	1	415756	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with candesartan alone increased cortical BZ ( 1 ) binding , and decreased ( 2 ) subunit mRNA expression in the cingulate cortex .
	manualset3
193501	2	415756	7	NULL	NULL	0	NULL	candesartan	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with candesartan alone increased cortical BZ ( 1 ) binding , and decreased ( 2 ) subunit mRNA expression in the cingulate cortex .
	manualset3
193502	3	415756	7	NULL	NULL	0	NULL	cortical BZ ( 1 ) binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with candesartan alone increased cortical BZ ( 1 ) binding , and decreased ( 2 ) subunit mRNA expression in the cingulate cortex .
	manualset3
193503	4	415756	7	NULL	NULL	0	NULL	subunit mRNA expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with candesartan alone increased cortical BZ ( 1 ) binding , and decreased ( 2 ) subunit mRNA expression in the cingulate cortex .
	manualset3
193504	5	415756	7	NULL	NULL	0	NULL	cingulate cortex 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with candesartan alone increased cortical BZ ( 1 ) binding , and decreased ( 2 ) subunit mRNA expression in the cingulate cortex .
	manualset3
193505	1	415757	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with dexamethasone , but not cAMP , reduced TGF-beta1 and - beta2 transcripts and TGF-beta bioactivity in culture medium .
	manualset3
193506	2	415757	7	NULL	NULL	0	NULL	dexamethasone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with dexamethasone , but not cAMP , reduced TGF-beta1 and - beta2 transcripts and TGF-beta bioactivity in culture medium .
	manualset3
193507	3	415757	7	NULL	NULL	0	NULL	cAMP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with dexamethasone , but not cAMP , reduced TGF-beta1 and - beta2 transcripts and TGF-beta bioactivity in culture medium .
	manualset3
193508	4	415757	7	NULL	NULL	0	NULL	TGF-beta1 transcripts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with dexamethasone , but not cAMP , reduced TGF-beta1 and - beta2 transcripts and TGF-beta bioactivity in culture medium .
	manualset3
193509	5	415757	7	NULL	NULL	0	NULL	TGF-beta2 transcripts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with dexamethasone , but not cAMP , reduced TGF-beta1 and - beta2 transcripts and TGF-beta bioactivity in culture medium .
	manualset3
193510	6	415757	7	NULL	NULL	0	NULL	TGF-beta bioactivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with dexamethasone , but not cAMP , reduced TGF-beta1 and - beta2 transcripts and TGF-beta bioactivity in culture medium .
	manualset3
193511	7	415757	7	NULL	NULL	0	NULL	culture medium	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with dexamethasone , but not cAMP , reduced TGF-beta1 and - beta2 transcripts and TGF-beta bioactivity in culture medium .
	manualset3
193512	1	415758	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with iron improved IQ scores significantly ; other studies found differential effects : improvement in cognition and mental scores in older but not in younger children .
	manualset3
193513	2	415758	7	NULL	NULL	0	NULL	iron	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with iron improved IQ scores significantly ; other studies found differential effects : improvement in cognition and mental scores in older but not in younger children .
	manualset3
193514	3	415758	7	NULL	NULL	0	NULL	 IQ scores	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with iron improved IQ scores significantly ; other studies found differential effects : improvement in cognition and mental scores in older but not in younger children .
	manualset3
193515	4	415758	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with iron improved IQ scores significantly ; other studies found differential effects : improvement in cognition and mental scores in older but not in younger children .
	manualset3
193516	5	415758	7	NULL	NULL	0	NULL	 differential effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with iron improved IQ scores significantly ; other studies found differential effects : improvement in cognition and mental scores in older but not in younger children .
	manualset3
193517	6	415758	7	NULL	NULL	0	NULL	improvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with iron improved IQ scores significantly ; other studies found differential effects : improvement in cognition and mental scores in older but not in younger children .
	manualset3
193518	7	415758	7	NULL	NULL	0	NULL	cognition scores	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with iron improved IQ scores significantly ; other studies found differential effects : improvement in cognition and mental scores in older but not in younger children .
	manualset3
193519	8	415758	7	NULL	NULL	0	NULL	mental scores	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with iron improved IQ scores significantly ; other studies found differential effects : improvement in cognition and mental scores in older but not in younger children .
	manualset3
193520	9	415758	7	NULL	NULL	0	NULL	younger children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with iron improved IQ scores significantly ; other studies found differential effects : improvement in cognition and mental scores in older but not in younger children .
	manualset3
193521	1	415759	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with morphine ( 1 or 5 mg/kg ) , but not pancuronium ( 0.3 mg/kg ) , attenuated the plasma beta-END-LI response to mechanical ventilation , suggesting that a subconscious phenomenon , perhaps related to pain , was partially responsible for the profound release of pituitary beta-END-LI associated with artificial respiration .
	manualset3
193522	2	415759	7	NULL	NULL	0	NULL	morphine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with morphine ( 1 or 5 mg/kg ) , but not pancuronium ( 0.3 mg/kg ) , attenuated the plasma beta-END-LI response to mechanical ventilation , suggesting that a subconscious phenomenon , perhaps related to pain , was partially responsible for the profound release of pituitary beta-END-LI associated with artificial respiration .
	manualset3
193523	3	415759	7	NULL	NULL	NULL	NULL	1 or 5 mg/kg	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Treatment with morphine ( 1 or 5 mg/kg ) , but not pancuronium ( 0.3 mg/kg ) , attenuated the plasma beta-END-LI response to mechanical ventilation , suggesting that a subconscious phenomenon , perhaps related to pain , was partially responsible for the profound release of pituitary beta-END-LI associated with artificial respiration .
	manualset3
193524	4	415759	7	NULL	NULL	0	NULL	pancuronium	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with morphine ( 1 or 5 mg/kg ) , but not pancuronium ( 0.3 mg/kg ) , attenuated the plasma beta-END-LI response to mechanical ventilation , suggesting that a subconscious phenomenon , perhaps related to pain , was partially responsible for the profound release of pituitary beta-END-LI associated with artificial respiration .
	manualset3
193525	5	415759	7	NULL	NULL	0	NULL	0.3 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with morphine ( 1 or 5 mg/kg ) , but not pancuronium ( 0.3 mg/kg ) , attenuated the plasma beta-END-LI response to mechanical ventilation , suggesting that a subconscious phenomenon , perhaps related to pain , was partially responsible for the profound release of pituitary beta-END-LI associated with artificial respiration .
	manualset3
193526	6	415759	7	NULL	NULL	0	NULL	plasma beta-END-LI response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with morphine ( 1 or 5 mg/kg ) , but not pancuronium ( 0.3 mg/kg ) , attenuated the plasma beta-END-LI response to mechanical ventilation , suggesting that a subconscious phenomenon , perhaps related to pain , was partially responsible for the profound release of pituitary beta-END-LI associated with artificial respiration .
	manualset3
193527	7	415759	7	NULL	NULL	0	NULL	mechanical ventilation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with morphine ( 1 or 5 mg/kg ) , but not pancuronium ( 0.3 mg/kg ) , attenuated the plasma beta-END-LI response to mechanical ventilation , suggesting that a subconscious phenomenon , perhaps related to pain , was partially responsible for the profound release of pituitary beta-END-LI associated with artificial respiration .
	manualset3
193528	8	415759	7	NULL	NULL	0	NULL	subconscious phenomenon	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with morphine ( 1 or 5 mg/kg ) , but not pancuronium ( 0.3 mg/kg ) , attenuated the plasma beta-END-LI response to mechanical ventilation , suggesting that a subconscious phenomenon , perhaps related to pain , was partially responsible for the profound release of pituitary beta-END-LI associated with artificial respiration .
	manualset3
193529	9	415759	7	NULL	NULL	0	NULL	pain 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with morphine ( 1 or 5 mg/kg ) , but not pancuronium ( 0.3 mg/kg ) , attenuated the plasma beta-END-LI response to mechanical ventilation , suggesting that a subconscious phenomenon , perhaps related to pain , was partially responsible for the profound release of pituitary beta-END-LI associated with artificial respiration .
	manualset3
193530	10	415759	7	NULL	NULL	0	NULL	release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with morphine ( 1 or 5 mg/kg ) , but not pancuronium ( 0.3 mg/kg ) , attenuated the plasma beta-END-LI response to mechanical ventilation , suggesting that a subconscious phenomenon , perhaps related to pain , was partially responsible for the profound release of pituitary beta-END-LI associated with artificial respiration .
	manualset3
193531	11	415759	7	NULL	NULL	0	NULL	pituitary beta-END-LI associated with artificial respiration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with morphine ( 1 or 5 mg/kg ) , but not pancuronium ( 0.3 mg/kg ) , attenuated the plasma beta-END-LI response to mechanical ventilation , suggesting that a subconscious phenomenon , perhaps related to pain , was partially responsible for the profound release of pituitary beta-END-LI associated with artificial respiration .
	manualset3
193532	1	415760	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with oral prednisolone was initiated and seemed to successfully resolve the vasculitis activity .
	manualset3
193533	2	415760	7	NULL	NULL	0	NULL	 oral prednisolone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with oral prednisolone was initiated and seemed to successfully resolve the vasculitis activity .
	manualset3
193534	3	415760	7	NULL	NULL	0	NULL	vasculitis activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with oral prednisolone was initiated and seemed to successfully resolve the vasculitis activity .
	manualset3
193535	1	415761	7	NULL	NULL	0	NULL	Treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with rHTNF first and then topoisomerase-targeted drugs yielded no enhanced cytotoxicity , whereas pretreatment with drug followed by rHTNF yielded marked enhancement of cytotoxicity .
	manualset3
193536	2	415761	7	NULL	NULL	0	NULL	 rHTNF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with rHTNF first and then topoisomerase-targeted drugs yielded no enhanced cytotoxicity , whereas pretreatment with drug followed by rHTNF yielded marked enhancement of cytotoxicity .
	manualset3
193537	3	415761	7	NULL	NULL	0	NULL	topoisomerase-targeted drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with rHTNF first and then topoisomerase-targeted drugs yielded no enhanced cytotoxicity , whereas pretreatment with drug followed by rHTNF yielded marked enhancement of cytotoxicity .
	manualset3
193538	4	415761	7	NULL	NULL	0	NULL	no enhanced cytotoxicity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with rHTNF first and then topoisomerase-targeted drugs yielded no enhanced cytotoxicity , whereas pretreatment with drug followed by rHTNF yielded marked enhancement of cytotoxicity .
	manualset3
193539	5	415761	7	NULL	NULL	0	NULL	pretreatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with rHTNF first and then topoisomerase-targeted drugs yielded no enhanced cytotoxicity , whereas pretreatment with drug followed by rHTNF yielded marked enhancement of cytotoxicity .
	manualset3
193540	6	415761	7	NULL	NULL	0	NULL	 drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with rHTNF first and then topoisomerase-targeted drugs yielded no enhanced cytotoxicity , whereas pretreatment with drug followed by rHTNF yielded marked enhancement of cytotoxicity .
	manualset3
193541	7	415761	7	NULL	NULL	0	NULL	rHTNF 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with rHTNF first and then topoisomerase-targeted drugs yielded no enhanced cytotoxicity , whereas pretreatment with drug followed by rHTNF yielded marked enhancement of cytotoxicity .
	manualset3
193542	8	415761	7	NULL	NULL	0	NULL	enhancement	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with rHTNF first and then topoisomerase-targeted drugs yielded no enhanced cytotoxicity , whereas pretreatment with drug followed by rHTNF yielded marked enhancement of cytotoxicity .
	manualset3
193543	9	415761	7	NULL	NULL	0	NULL	cytotoxicity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with rHTNF first and then topoisomerase-targeted drugs yielded no enhanced cytotoxicity , whereas pretreatment with drug followed by rHTNF yielded marked enhancement of cytotoxicity .
	manualset3
193544	1	415762	7	NULL	NULL	0	NULL	Treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with tablets was slightly but significantly more effective than capsules .
	manualset3
193545	2	415762	7	NULL	NULL	0	NULL	 tablets	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with tablets was slightly but significantly more effective than capsules .
	manualset3
193546	3	415762	7	NULL	NULL	0	NULL	capsules	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with tablets was slightly but significantly more effective than capsules .
	manualset3
193547	1	415763	7	NULL	NULL	0	NULL	chamber	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	After leaving the chamber ( day 3 , 10-h fast ) , IS was measured by a 2-h clamp ( 120 mU/m ( 2 ) / min ) .
	manualset3
193548	2	415763	7	NULL	NULL	0	NULL	day 3	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After leaving the chamber ( day 3 , 10-h fast ) , IS was measured by a 2-h clamp ( 120 mU/m ( 2 ) / min ) .
	manualset3
193549	3	415763	7	NULL	NULL	0	NULL	10-h fast	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After leaving the chamber ( day 3 , 10-h fast ) , IS was measured by a 2-h clamp ( 120 mU/m ( 2 ) / min ) .
	manualset3
193550	4	415763	7	NULL	NULL	0	NULL	IS 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After leaving the chamber ( day 3 , 10-h fast ) , IS was measured by a 2-h clamp ( 120 mU/m ( 2 ) / min ) .
	manualset3
193551	5	415763	7	NULL	NULL	0	NULL	2-h clamp	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After leaving the chamber ( day 3 , 10-h fast ) , IS was measured by a 2-h clamp ( 120 mU/m ( 2 ) / min ) .
	manualset3
193552	6	415763	7	NULL	NULL	0	NULL	120 mU/m ( 2 ) / min	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	After leaving the chamber ( day 3 , 10-h fast ) , IS was measured by a 2-h clamp ( 120 mU/m ( 2 ) / min ) .
	manualset3
193553	1	415764	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with the glucocorticoid receptor antagonist , RU 486 , however , did not prevent cell loss in the bone marrow of mice exposed to the mixture of propanil and 2 , 4-D .
	manualset3
193554	2	415764	7	NULL	NULL	0	NULL	glucocorticoid receptor antagonist	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with the glucocorticoid receptor antagonist , RU 486 , however , did not prevent cell loss in the bone marrow of mice exposed to the mixture of propanil and 2 , 4-D .
	manualset3
193555	3	415764	7	NULL	NULL	0	NULL	RU 486	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with the glucocorticoid receptor antagonist , RU 486 , however , did not prevent cell loss in the bone marrow of mice exposed to the mixture of propanil and 2 , 4-D .
	manualset3
193556	4	415764	7	NULL	NULL	0	NULL	cell loss	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with the glucocorticoid receptor antagonist , RU 486 , however , did not prevent cell loss in the bone marrow of mice exposed to the mixture of propanil and 2 , 4-D .
	manualset3
193557	5	415764	7	NULL	NULL	0	NULL	bone marrow	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with the glucocorticoid receptor antagonist , RU 486 , however , did not prevent cell loss in the bone marrow of mice exposed to the mixture of propanil and 2 , 4-D .
	manualset3
193558	6	415764	7	NULL	NULL	0	NULL	 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with the glucocorticoid receptor antagonist , RU 486 , however , did not prevent cell loss in the bone marrow of mice exposed to the mixture of propanil and 2 , 4-D .
	manualset3
193559	7	415764	7	NULL	NULL	0	NULL	 mixture	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with the glucocorticoid receptor antagonist , RU 486 , however , did not prevent cell loss in the bone marrow of mice exposed to the mixture of propanil and 2 , 4-D .
	manualset3
193560	8	415764	7	NULL	NULL	0	NULL	propanil 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with the glucocorticoid receptor antagonist , RU 486 , however , did not prevent cell loss in the bone marrow of mice exposed to the mixture of propanil and 2 , 4-D .
	manualset3
193561	9	415764	7	NULL	NULL	0	NULL	2 , 4-D	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with the glucocorticoid receptor antagonist , RU 486 , however , did not prevent cell loss in the bone marrow of mice exposed to the mixture of propanil and 2 , 4-D .
	manualset3
193562	1	415765	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with the liver X receptor ligand 22-OH increased efflux to apoA-I in AcLDL-loaded but not LDL-loaded cells .
	manualset3
193563	2	415765	7	NULL	NULL	0	NULL	liver X receptor ligand	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with the liver X receptor ligand 22-OH increased efflux to apoA-I in AcLDL-loaded but not LDL-loaded cells .
	manualset3
193564	3	415765	7	NULL	NULL	0	NULL	22-OH	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with the liver X receptor ligand 22-OH increased efflux to apoA-I in AcLDL-loaded but not LDL-loaded cells .
	manualset3
193565	4	415765	7	NULL	NULL	0	NULL	efflux	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with the liver X receptor ligand 22-OH increased efflux to apoA-I in AcLDL-loaded but not LDL-loaded cells .
	manualset3
193566	5	415765	7	NULL	NULL	0	NULL	apoA-I	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with the liver X receptor ligand 22-OH increased efflux to apoA-I in AcLDL-loaded but not LDL-loaded cells .
	manualset3
193567	6	415765	7	NULL	NULL	0	NULL	AcLDL-loaded cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with the liver X receptor ligand 22-OH increased efflux to apoA-I in AcLDL-loaded but not LDL-loaded cells .
	manualset3
193568	7	415765	7	NULL	NULL	0	NULL	LDL-loaded cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with the liver X receptor ligand 22-OH increased efflux to apoA-I in AcLDL-loaded but not LDL-loaded cells .
	manualset3
193569	1	415766	7	NULL	NULL	0	NULL	Treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with threo-beta-F-Asn ( 5-10 mM ) resulted in : 1 ) a reduction in the amount of the more highly glycosylated form of POMC ( Mr = 32 , 000 ) relative to the less glycosylated form ( Mr = 29 , 000 ) and 2 ) the appearance of a new species of POMC ( Mr = 27 , 000 ) .
	manualset3
193570	2	415766	7	NULL	NULL	NULL	NULL	threo-beta-F-Asn	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Treatment with threo-beta-F-Asn ( 5-10 mM ) resulted in : 1 ) a reduction in the amount of the more highly glycosylated form of POMC ( Mr = 32 , 000 ) relative to the less glycosylated form ( Mr = 29 , 000 ) and 2 ) the appearance of a new species of POMC ( Mr = 27 , 000 ) .
	manualset3
193571	3	415766	7	NULL	NULL	0	NULL	5-10 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with threo-beta-F-Asn ( 5-10 mM ) resulted in : 1 ) a reduction in the amount of the more highly glycosylated form of POMC ( Mr = 32 , 000 ) relative to the less glycosylated form ( Mr = 29 , 000 ) and 2 ) the appearance of a new species of POMC ( Mr = 27 , 000 ) .
	manualset3
193572	4	415766	7	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with threo-beta-F-Asn ( 5-10 mM ) resulted in : 1 ) a reduction in the amount of the more highly glycosylated form of POMC ( Mr = 32 , 000 ) relative to the less glycosylated form ( Mr = 29 , 000 ) and 2 ) the appearance of a new species of POMC ( Mr = 27 , 000 ) .
	manualset3
193573	5	415766	7	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with threo-beta-F-Asn ( 5-10 mM ) resulted in : 1 ) a reduction in the amount of the more highly glycosylated form of POMC ( Mr = 32 , 000 ) relative to the less glycosylated form ( Mr = 29 , 000 ) and 2 ) the appearance of a new species of POMC ( Mr = 27 , 000 ) .
	manualset3
193574	6	415766	7	NULL	NULL	0	NULL	highly glycosylated form	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with threo-beta-F-Asn ( 5-10 mM ) resulted in : 1 ) a reduction in the amount of the more highly glycosylated form of POMC ( Mr = 32 , 000 ) relative to the less glycosylated form ( Mr = 29 , 000 ) and 2 ) the appearance of a new species of POMC ( Mr = 27 , 000 ) .
	manualset3
193575	7	415766	7	NULL	NULL	0	NULL	POMC	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with threo-beta-F-Asn ( 5-10 mM ) resulted in : 1 ) a reduction in the amount of the more highly glycosylated form of POMC ( Mr = 32 , 000 ) relative to the less glycosylated form ( Mr = 29 , 000 ) and 2 ) the appearance of a new species of POMC ( Mr = 27 , 000 ) .
	manualset3
193576	8	415766	7	NULL	NULL	0	NULL	Mr = 32 , 000	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with threo-beta-F-Asn ( 5-10 mM ) resulted in : 1 ) a reduction in the amount of the more highly glycosylated form of POMC ( Mr = 32 , 000 ) relative to the less glycosylated form ( Mr = 29 , 000 ) and 2 ) the appearance of a new species of POMC ( Mr = 27 , 000 ) .
	manualset3
193577	9	415766	7	NULL	NULL	0	NULL	 less glycosylated form	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with threo-beta-F-Asn ( 5-10 mM ) resulted in : 1 ) a reduction in the amount of the more highly glycosylated form of POMC ( Mr = 32 , 000 ) relative to the less glycosylated form ( Mr = 29 , 000 ) and 2 ) the appearance of a new species of POMC ( Mr = 27 , 000 ) .
	manualset3
193578	10	415766	7	NULL	NULL	0	NULL	Mr = 29 , 000	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with threo-beta-F-Asn ( 5-10 mM ) resulted in : 1 ) a reduction in the amount of the more highly glycosylated form of POMC ( Mr = 32 , 000 ) relative to the less glycosylated form ( Mr = 29 , 000 ) and 2 ) the appearance of a new species of POMC ( Mr = 27 , 000 ) .
	manualset3
193579	11	415766	7	NULL	NULL	0	NULL	appearance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with threo-beta-F-Asn ( 5-10 mM ) resulted in : 1 ) a reduction in the amount of the more highly glycosylated form of POMC ( Mr = 32 , 000 ) relative to the less glycosylated form ( Mr = 29 , 000 ) and 2 ) the appearance of a new species of POMC ( Mr = 27 , 000 ) .
	manualset3
193580	12	415766	7	NULL	NULL	0	NULL	new species 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with threo-beta-F-Asn ( 5-10 mM ) resulted in : 1 ) a reduction in the amount of the more highly glycosylated form of POMC ( Mr = 32 , 000 ) relative to the less glycosylated form ( Mr = 29 , 000 ) and 2 ) the appearance of a new species of POMC ( Mr = 27 , 000 ) .
	manualset3
193581	13	415766	7	NULL	NULL	0	NULL	POMC 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with threo-beta-F-Asn ( 5-10 mM ) resulted in : 1 ) a reduction in the amount of the more highly glycosylated form of POMC ( Mr = 32 , 000 ) relative to the less glycosylated form ( Mr = 29 , 000 ) and 2 ) the appearance of a new species of POMC ( Mr = 27 , 000 ) .
	manualset3
193582	14	415766	7	NULL	NULL	0	NULL	Mr = 27 , 000	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with threo-beta-F-Asn ( 5-10 mM ) resulted in : 1 ) a reduction in the amount of the more highly glycosylated form of POMC ( Mr = 32 , 000 ) relative to the less glycosylated form ( Mr = 29 , 000 ) and 2 ) the appearance of a new species of POMC ( Mr = 27 , 000 ) .
	manualset3
193583	1	415767	7	NULL	NULL	0	NULL	Treatments	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatments with estrogen , estrogen plus bromocryptine , and perphenazine plus tamoxifen but not perphenazine alone were able to partially restore PGRs although this effect was of borderline statistical significance .
	manualset3
193584	2	415767	7	NULL	NULL	0	NULL	estrogen	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatments with estrogen , estrogen plus bromocryptine , and perphenazine plus tamoxifen but not perphenazine alone were able to partially restore PGRs although this effect was of borderline statistical significance .
	manualset3
193585	3	415767	7	NULL	NULL	NULL	NULL	estrogen plus bromocryptine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Treatments with estrogen , estrogen plus bromocryptine , and perphenazine plus tamoxifen but not perphenazine alone were able to partially restore PGRs although this effect was of borderline statistical significance .
	manualset3
193586	4	415767	7	NULL	NULL	0	NULL	perphenazine plus tamoxifen	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatments with estrogen , estrogen plus bromocryptine , and perphenazine plus tamoxifen but not perphenazine alone were able to partially restore PGRs although this effect was of borderline statistical significance .
	manualset3
193587	5	415767	7	NULL	NULL	0	NULL	perphenazine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatments with estrogen , estrogen plus bromocryptine , and perphenazine plus tamoxifen but not perphenazine alone were able to partially restore PGRs although this effect was of borderline statistical significance .
	manualset3
193588	6	415767	7	NULL	NULL	0	NULL	PGRs	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatments with estrogen , estrogen plus bromocryptine , and perphenazine plus tamoxifen but not perphenazine alone were able to partially restore PGRs although this effect was of borderline statistical significance .
	manualset3
193589	7	415767	7	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatments with estrogen , estrogen plus bromocryptine , and perphenazine plus tamoxifen but not perphenazine alone were able to partially restore PGRs although this effect was of borderline statistical significance .
	manualset3
193590	8	415767	7	NULL	NULL	0	NULL	statistical significance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatments with estrogen , estrogen plus bromocryptine , and perphenazine plus tamoxifen but not perphenazine alone were able to partially restore PGRs although this effect was of borderline statistical significance .
	manualset3
193591	1	415768	7	NULL	NULL	0	NULL	Trends	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Trends in ( CO ( 2 ) ) ( INT ) throughout the stress cycle indicated nonstomatal effects of water stress on CO ( 2 ) exchange rate were greater in high N plants .
	manualset3
193592	2	415768	7	NULL	NULL	0	NULL	 ( CO ( 2 ) ) ( INT )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Trends in ( CO ( 2 ) ) ( INT ) throughout the stress cycle indicated nonstomatal effects of water stress on CO ( 2 ) exchange rate were greater in high N plants .
	manualset3
193593	3	415768	7	NULL	NULL	0	NULL	stress cycle 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Trends in ( CO ( 2 ) ) ( INT ) throughout the stress cycle indicated nonstomatal effects of water stress on CO ( 2 ) exchange rate were greater in high N plants .
	manualset3
193594	4	415768	7	NULL	NULL	0	NULL	nonstomatal effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Trends in ( CO ( 2 ) ) ( INT ) throughout the stress cycle indicated nonstomatal effects of water stress on CO ( 2 ) exchange rate were greater in high N plants .
	manualset3
193595	5	415768	7	NULL	NULL	0	NULL	water stress	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Trends in ( CO ( 2 ) ) ( INT ) throughout the stress cycle indicated nonstomatal effects of water stress on CO ( 2 ) exchange rate were greater in high N plants .
	manualset3
193596	6	415768	7	NULL	NULL	0	NULL	CO ( 2 ) exchange rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Trends in ( CO ( 2 ) ) ( INT ) throughout the stress cycle indicated nonstomatal effects of water stress on CO ( 2 ) exchange rate were greater in high N plants .
	manualset3
193597	7	415768	7	NULL	NULL	0	NULL	high N plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Trends in ( CO ( 2 ) ) ( INT ) throughout the stress cycle indicated nonstomatal effects of water stress on CO ( 2 ) exchange rate were greater in high N plants .
	manualset3
193598	1	415769	7	NULL	NULL	0	NULL	Trends	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Trends in eczema in the first 18 years of life : results from the Isle of Wight 1989 birth cohort study .
	manualset3
193599	2	415769	7	NULL	NULL	0	NULL	eczema 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Trends in eczema in the first 18 years of life : results from the Isle of Wight 1989 birth cohort study .
	manualset3
193600	3	415769	7	NULL	NULL	0	NULL	 first 18 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Trends in eczema in the first 18 years of life : results from the Isle of Wight 1989 birth cohort study .
	manualset3
193601	4	415769	7	NULL	NULL	0	NULL	life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Trends in eczema in the first 18 years of life : results from the Isle of Wight 1989 birth cohort study .
	manualset3
193602	5	415769	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Trends in eczema in the first 18 years of life : results from the Isle of Wight 1989 birth cohort study .
	manualset3
193603	6	415769	7	NULL	NULL	0	NULL	Isle of Wight 1989 birth cohort study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Trends in eczema in the first 18 years of life : results from the Isle of Wight 1989 birth cohort study .
	manualset3
193604	1	415770	7	NULL	NULL	0	NULL	Trends	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Trends in health service delivery for cataract surgery at a large Australian ophthalmic hospital .
	manualset3
193605	2	415770	7	NULL	NULL	0	NULL	health service delivery	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Trends in health service delivery for cataract surgery at a large Australian ophthalmic hospital .
	manualset3
193606	3	415770	7	NULL	NULL	0	NULL	 cataract surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Trends in health service delivery for cataract surgery at a large Australian ophthalmic hospital .
	manualset3
193607	4	415770	7	NULL	NULL	0	NULL	large Australian ophthalmic hospital	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Trends in health service delivery for cataract surgery at a large Australian ophthalmic hospital .
	manualset3
193608	1	415771	7	NULL	NULL	0	NULL	Trends	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Trends in resource utilization by children with neurological impairment in the United States inpatient health care system : a repeat cross-sectional study .
	manualset3
193609	2	415771	7	NULL	NULL	NULL	NULL	resource utilization	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Trends in resource utilization by children with neurological impairment in the United States inpatient health care system : a repeat cross-sectional study .
	manualset3
193610	3	415771	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Trends in resource utilization by children with neurological impairment in the United States inpatient health care system : a repeat cross-sectional study .
	manualset3
193611	4	415771	7	NULL	NULL	0	NULL	neurological impairment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Trends in resource utilization by children with neurological impairment in the United States inpatient health care system : a repeat cross-sectional study .
	manualset3
193612	5	415771	7	NULL	NULL	0	NULL	United States inpatient health care system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Trends in resource utilization by children with neurological impairment in the United States inpatient health care system : a repeat cross-sectional study .
	manualset3
193613	6	415771	7	NULL	NULL	0	NULL	repeat cross-sectional study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Trends in resource utilization by children with neurological impairment in the United States inpatient health care system : a repeat cross-sectional study .
	manualset3
193614	1	415772	7	NULL	NULL	0	NULL	Trends	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Trends in surgical treatment of breast cancer at an urban teaching hospital : a six-year review .
	manualset3
193615	2	415772	7	NULL	NULL	0	NULL	surgical treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Trends in surgical treatment of breast cancer at an urban teaching hospital : a six-year review .
	manualset3
193616	3	415772	7	NULL	NULL	0	NULL	breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Trends in surgical treatment of breast cancer at an urban teaching hospital : a six-year review .
	manualset3
193617	4	415772	7	NULL	NULL	0	NULL	urban teaching hospital	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Trends in surgical treatment of breast cancer at an urban teaching hospital : a six-year review .
	manualset3
193618	5	415772	7	NULL	NULL	0	NULL	six-year review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Trends in surgical treatment of breast cancer at an urban teaching hospital : a six-year review .
	manualset3
193619	1	415773	7	NULL	NULL	0	NULL	liquid-liquid extraction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After liquid-liquid extraction and derivatization with phosgene in an aqueous pH 10.1 buffer , the cyclic oxazolidone derivative is quantitated with a clenbuterol analog as internal standard ( NAB-760 Cl ) .
	manualset3
193620	2	415773	7	NULL	NULL	0	NULL	derivatization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After liquid-liquid extraction and derivatization with phosgene in an aqueous pH 10.1 buffer , the cyclic oxazolidone derivative is quantitated with a clenbuterol analog as internal standard ( NAB-760 Cl ) .
	manualset3
193621	3	415773	7	NULL	NULL	0	NULL	phosgene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After liquid-liquid extraction and derivatization with phosgene in an aqueous pH 10.1 buffer , the cyclic oxazolidone derivative is quantitated with a clenbuterol analog as internal standard ( NAB-760 Cl ) .
	manualset3
193622	4	415773	7	NULL	NULL	0	NULL	aqueous pH 10.1 buffer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After liquid-liquid extraction and derivatization with phosgene in an aqueous pH 10.1 buffer , the cyclic oxazolidone derivative is quantitated with a clenbuterol analog as internal standard ( NAB-760 Cl ) .
	manualset3
193623	5	415773	7	NULL	NULL	0	NULL	cyclic oxazolidone derivative	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After liquid-liquid extraction and derivatization with phosgene in an aqueous pH 10.1 buffer , the cyclic oxazolidone derivative is quantitated with a clenbuterol analog as internal standard ( NAB-760 Cl ) .
	manualset3
193624	6	415773	7	NULL	NULL	0	NULL	clenbuterol analog	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After liquid-liquid extraction and derivatization with phosgene in an aqueous pH 10.1 buffer , the cyclic oxazolidone derivative is quantitated with a clenbuterol analog as internal standard ( NAB-760 Cl ) .
	manualset3
193625	7	415773	7	NULL	NULL	0	NULL	internal standard	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After liquid-liquid extraction and derivatization with phosgene in an aqueous pH 10.1 buffer , the cyclic oxazolidone derivative is quantitated with a clenbuterol analog as internal standard ( NAB-760 Cl ) .
	manualset3
193626	8	415773	7	NULL	NULL	0	NULL	NAB-760 Cl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After liquid-liquid extraction and derivatization with phosgene in an aqueous pH 10.1 buffer , the cyclic oxazolidone derivative is quantitated with a clenbuterol analog as internal standard ( NAB-760 Cl ) .
	manualset3
193627	1	415774	7	NULL	NULL	0	NULL	Triage and Injury Severity Scores	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Triage and Injury Severity Scores as predictors of mortality and hospital admission for injuries : a validation study .
	manualset3
193628	2	415774	7	NULL	NULL	0	NULL	predictors 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Triage and Injury Severity Scores as predictors of mortality and hospital admission for injuries : a validation study .
	manualset3
193629	3	415774	7	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Triage and Injury Severity Scores as predictors of mortality and hospital admission for injuries : a validation study .
	manualset3
193630	4	415774	7	NULL	NULL	0	NULL	hospital admission	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Triage and Injury Severity Scores as predictors of mortality and hospital admission for injuries : a validation study .
	manualset3
193631	5	415774	7	NULL	NULL	0	NULL	 injuries	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Triage and Injury Severity Scores as predictors of mortality and hospital admission for injuries : a validation study .
	manualset3
193632	6	415774	7	NULL	NULL	0	NULL	validation study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Triage and Injury Severity Scores as predictors of mortality and hospital admission for injuries : a validation study .
	manualset3
193633	1	415775	7	NULL	NULL	0	NULL	Trial registration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Trial registration and wandering outcomes .
	manualset3
193634	2	415775	7	NULL	NULL	0	NULL	wandering outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Trial registration and wandering outcomes .
	manualset3
193635	1	415776	7	NULL	NULL	0	NULL	Tribology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Tribology is the branch of engineering that deals with the interaction of surfaces in relative motion ( as in bearings or gears ) : their design , friction , adhesion , lubrication and wear .
	manualset3
193636	2	415776	7	NULL	NULL	0	NULL	branch	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Tribology is the branch of engineering that deals with the interaction of surfaces in relative motion ( as in bearings or gears ) : their design , friction , adhesion , lubrication and wear .
	manualset3
193637	3	415776	7	NULL	NULL	0	NULL	engineering	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Tribology is the branch of engineering that deals with the interaction of surfaces in relative motion ( as in bearings or gears ) : their design , friction , adhesion , lubrication and wear .
	manualset3
193638	4	415776	7	NULL	NULL	0	NULL	 interaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Tribology is the branch of engineering that deals with the interaction of surfaces in relative motion ( as in bearings or gears ) : their design , friction , adhesion , lubrication and wear .
	manualset3
193639	5	415776	7	NULL	NULL	0	NULL	surfaces	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Tribology is the branch of engineering that deals with the interaction of surfaces in relative motion ( as in bearings or gears ) : their design , friction , adhesion , lubrication and wear .
	manualset3
193640	6	415776	7	NULL	NULL	0	NULL	relative motion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Tribology is the branch of engineering that deals with the interaction of surfaces in relative motion ( as in bearings or gears ) : their design , friction , adhesion , lubrication and wear .
	manualset3
193641	7	415776	7	NULL	NULL	0	NULL	bearings	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Tribology is the branch of engineering that deals with the interaction of surfaces in relative motion ( as in bearings or gears ) : their design , friction , adhesion , lubrication and wear .
	manualset3
193642	8	415776	7	NULL	NULL	0	NULL	gears	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Tribology is the branch of engineering that deals with the interaction of surfaces in relative motion ( as in bearings or gears ) : their design , friction , adhesion , lubrication and wear .
	manualset3
193643	9	415776	7	NULL	NULL	NULL	NULL	design	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Tribology is the branch of engineering that deals with the interaction of surfaces in relative motion ( as in bearings or gears ) : their design , friction , adhesion , lubrication and wear .
	manualset3
193644	10	415776	7	NULL	NULL	0	NULL	friction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Tribology is the branch of engineering that deals with the interaction of surfaces in relative motion ( as in bearings or gears ) : their design , friction , adhesion , lubrication and wear .
	manualset3
193645	11	415776	7	NULL	NULL	0	NULL	adhesion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Tribology is the branch of engineering that deals with the interaction of surfaces in relative motion ( as in bearings or gears ) : their design , friction , adhesion , lubrication and wear .
	manualset3
193646	12	415776	7	NULL	NULL	0	NULL	lubrication	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Tribology is the branch of engineering that deals with the interaction of surfaces in relative motion ( as in bearings or gears ) : their design , friction , adhesion , lubrication and wear .
	manualset3
193647	13	415776	7	NULL	NULL	0	NULL	wear	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Tribology is the branch of engineering that deals with the interaction of surfaces in relative motion ( as in bearings or gears ) : their design , friction , adhesion , lubrication and wear .
	manualset3
193648	1	415777	7	NULL	NULL	0	NULL	Trichoblastic carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Trichoblastic carcinoma ( or malignant trichoblastoma ) is a rare malignant cancer of adnexal structures with morphological features that in some cases are reminiscent of a trichoblastoma .
	manualset3
193649	2	415777	7	NULL	NULL	0	NULL	malignant trichoblastoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Trichoblastic carcinoma ( or malignant trichoblastoma ) is a rare malignant cancer of adnexal structures with morphological features that in some cases are reminiscent of a trichoblastoma .
	manualset3
193650	3	415777	7	NULL	NULL	0	NULL	malignant cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Trichoblastic carcinoma ( or malignant trichoblastoma ) is a rare malignant cancer of adnexal structures with morphological features that in some cases are reminiscent of a trichoblastoma .
	manualset3
193651	4	415777	7	NULL	NULL	0	NULL	adnexal structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Trichoblastic carcinoma ( or malignant trichoblastoma ) is a rare malignant cancer of adnexal structures with morphological features that in some cases are reminiscent of a trichoblastoma .
	manualset3
193652	5	415777	7	NULL	NULL	0	NULL	morphological features	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Trichoblastic carcinoma ( or malignant trichoblastoma ) is a rare malignant cancer of adnexal structures with morphological features that in some cases are reminiscent of a trichoblastoma .
	manualset3
193653	6	415777	7	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Trichoblastic carcinoma ( or malignant trichoblastoma ) is a rare malignant cancer of adnexal structures with morphological features that in some cases are reminiscent of a trichoblastoma .
	manualset3
193654	7	415777	7	NULL	NULL	0	NULL	 trichoblastoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Trichoblastic carcinoma ( or malignant trichoblastoma ) is a rare malignant cancer of adnexal structures with morphological features that in some cases are reminiscent of a trichoblastoma .
	manualset3
193655	1	415778	7	NULL	NULL	0	NULL	Trichogenic trichoblastoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Trichogenic trichoblastoma arising on the supraclavicular fossa with an immunohistochemical study of cytokeratin expression .
	manualset3
193656	2	415778	7	NULL	NULL	0	NULL	supraclavicular fossa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Trichogenic trichoblastoma arising on the supraclavicular fossa with an immunohistochemical study of cytokeratin expression .
	manualset3
193657	3	415778	7	NULL	NULL	0	NULL	immunohistochemical study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Trichogenic trichoblastoma arising on the supraclavicular fossa with an immunohistochemical study of cytokeratin expression .
	manualset3
193658	4	415778	7	NULL	NULL	0	NULL	cytokeratin expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Trichogenic trichoblastoma arising on the supraclavicular fossa with an immunohistochemical study of cytokeratin expression .
	manualset3
193659	1	415779	7	NULL	NULL	0	NULL	Trigger fingers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Trigger fingers took significantly longer for the symptoms to subside .
	manualset3
193660	2	415779	7	NULL	NULL	0	NULL	symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Trigger fingers took significantly longer for the symptoms to subside .
	manualset3
193661	1	415780	7	NULL	NULL	0	NULL	Triiodothyronine radioimmunoassay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Triiodothyronine radioimmunoassay and its application to thyroid disorders .
	manualset3
193662	2	415780	7	NULL	NULL	0	NULL	application	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Triiodothyronine radioimmunoassay and its application to thyroid disorders .
	manualset3
193663	3	415780	7	NULL	NULL	0	NULL	thyroid disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Triiodothyronine radioimmunoassay and its application to thyroid disorders .
	manualset3
193664	1	415781	7	NULL	NULL	0	NULL	Trilostane 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Trilostane is a competitive inhibitor of 3 beta-hydroxysteroid dehydrogenase activity in vitro and an orally active inhibitor of steroidogenesis in vivo .
	manualset3
193665	2	415781	7	NULL	NULL	0	NULL	competitive inhibitor	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Trilostane is a competitive inhibitor of 3 beta-hydroxysteroid dehydrogenase activity in vitro and an orally active inhibitor of steroidogenesis in vivo .
	manualset3
193666	3	415781	7	NULL	NULL	0	NULL	3 beta-hydroxysteroid dehydrogenase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Trilostane is a competitive inhibitor of 3 beta-hydroxysteroid dehydrogenase activity in vitro and an orally active inhibitor of steroidogenesis in vivo .
	manualset3
193667	4	415781	7	NULL	NULL	NULL	NULL	orally active inhibitor 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Trilostane is a competitive inhibitor of 3 beta-hydroxysteroid dehydrogenase activity in vitro and an orally active inhibitor of steroidogenesis in vivo .
	manualset3
193668	5	415781	7	NULL	NULL	0	NULL	steroidogenesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Trilostane is a competitive inhibitor of 3 beta-hydroxysteroid dehydrogenase activity in vitro and an orally active inhibitor of steroidogenesis in vivo .
	manualset3
193669	1	415782	7	NULL	NULL	0	NULL	Troglitazone ( CS-045 )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Troglitazone ( CS-045 ) is a new type of antidiabetic agent that decreases plasma glucose by enhancing insulin action in insulin-resistant diabetic animals and non-insulin-dependent diabetes mellitus ( NIDDM ) patients .
	manualset3
193670	2	415782	7	NULL	NULL	0	NULL	new type	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Troglitazone ( CS-045 ) is a new type of antidiabetic agent that decreases plasma glucose by enhancing insulin action in insulin-resistant diabetic animals and non-insulin-dependent diabetes mellitus ( NIDDM ) patients .
	manualset3
193671	3	415782	7	NULL	NULL	0	NULL	antidiabetic agent	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Troglitazone ( CS-045 ) is a new type of antidiabetic agent that decreases plasma glucose by enhancing insulin action in insulin-resistant diabetic animals and non-insulin-dependent diabetes mellitus ( NIDDM ) patients .
	manualset3
193672	4	415782	7	NULL	NULL	NULL	NULL	plasma glucose	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Troglitazone ( CS-045 ) is a new type of antidiabetic agent that decreases plasma glucose by enhancing insulin action in insulin-resistant diabetic animals and non-insulin-dependent diabetes mellitus ( NIDDM ) patients .
	manualset3
193673	5	415782	7	NULL	NULL	0	NULL	insulin action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Troglitazone ( CS-045 ) is a new type of antidiabetic agent that decreases plasma glucose by enhancing insulin action in insulin-resistant diabetic animals and non-insulin-dependent diabetes mellitus ( NIDDM ) patients .
	manualset3
193674	6	415782	7	NULL	NULL	0	NULL	insulin-resistant diabetic animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Troglitazone ( CS-045 ) is a new type of antidiabetic agent that decreases plasma glucose by enhancing insulin action in insulin-resistant diabetic animals and non-insulin-dependent diabetes mellitus ( NIDDM ) patients .
	manualset3
193675	7	415782	7	NULL	NULL	0	NULL	non-insulin-dependent diabetes mellitus ( NIDDM ) patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Troglitazone ( CS-045 ) is a new type of antidiabetic agent that decreases plasma glucose by enhancing insulin action in insulin-resistant diabetic animals and non-insulin-dependent diabetes mellitus ( NIDDM ) patients .
	manualset3
193676	1	415783	7	NULL	NULL	0	NULL	Tropical splenomegaly 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Tropical splenomegaly is thought to encompass a variety of diseases , most of them presenting an intermediate stage of reactive to autonome disorders of the lymphatic system .
	manualset3
193677	2	415783	7	NULL	NULL	0	NULL	diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Tropical splenomegaly is thought to encompass a variety of diseases , most of them presenting an intermediate stage of reactive to autonome disorders of the lymphatic system .
	manualset3
193678	3	415783	7	NULL	NULL	0	NULL	 intermediate stage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Tropical splenomegaly is thought to encompass a variety of diseases , most of them presenting an intermediate stage of reactive to autonome disorders of the lymphatic system .
	manualset3
193679	4	415783	7	NULL	NULL	0	NULL	autonome disorders 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Tropical splenomegaly is thought to encompass a variety of diseases , most of them presenting an intermediate stage of reactive to autonome disorders of the lymphatic system .
	manualset3
193680	5	415783	7	NULL	NULL	0	NULL	 lymphatic system 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Tropical splenomegaly is thought to encompass a variety of diseases , most of them presenting an intermediate stage of reactive to autonome disorders of the lymphatic system .
	manualset3
193681	1	415784	7	NULL	NULL	0	NULL	True vaginal prolapse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	True vaginal prolapse may occur near parturition , as the concentration of serum progesterone declines and the concentration of serum estrogen increases .
	manualset3
193682	2	415784	7	NULL	NULL	0	NULL	parturition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	True vaginal prolapse may occur near parturition , as the concentration of serum progesterone declines and the concentration of serum estrogen increases .
	manualset3
193683	3	415784	7	NULL	NULL	0	NULL	concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	True vaginal prolapse may occur near parturition , as the concentration of serum progesterone declines and the concentration of serum estrogen increases .
	manualset3
193684	4	415784	7	NULL	NULL	0	NULL	serum progesterone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	True vaginal prolapse may occur near parturition , as the concentration of serum progesterone declines and the concentration of serum estrogen increases .
	manualset3
193685	5	415784	7	NULL	NULL	0	NULL	concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	True vaginal prolapse may occur near parturition , as the concentration of serum progesterone declines and the concentration of serum estrogen increases .
	manualset3
193686	6	415784	7	NULL	NULL	0	NULL	serum estrogen	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	True vaginal prolapse may occur near parturition , as the concentration of serum progesterone declines and the concentration of serum estrogen increases .
	manualset3
193687	1	415785	7	NULL	NULL	0	NULL	Truncation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Truncation of the 49-residue sequence at its N or C terminus caused loss of inhibitory activity .
	manualset3
193688	2	415785	7	NULL	NULL	0	NULL	49-residue sequence	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Truncation of the 49-residue sequence at its N or C terminus caused loss of inhibitory activity .
	manualset3
193689	3	415785	7	NULL	NULL	0	NULL	N terminus	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Truncation of the 49-residue sequence at its N or C terminus caused loss of inhibitory activity .
	manualset3
193690	4	415785	7	NULL	NULL	0	NULL	C terminus	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Truncation of the 49-residue sequence at its N or C terminus caused loss of inhibitory activity .
	manualset3
193691	5	415785	7	NULL	NULL	0	NULL	inhibitory activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Truncation of the 49-residue sequence at its N or C terminus caused loss of inhibitory activity .
	manualset3
193692	1	415786	7	NULL	NULL	0	NULL	Trypanosoma brucei rhodesiense	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Trypanosoma brucei rhodesiense : mechanical transmission by tsetse , Glossina morsitans ( Diptera : Glossinidae ) , in the laboratory .
	manualset3
193693	2	415786	7	NULL	NULL	0	NULL	mechanical transmission	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Trypanosoma brucei rhodesiense : mechanical transmission by tsetse , Glossina morsitans ( Diptera : Glossinidae ) , in the laboratory .
	manualset3
193694	3	415786	7	NULL	NULL	0	NULL	tsetse	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Trypanosoma brucei rhodesiense : mechanical transmission by tsetse , Glossina morsitans ( Diptera : Glossinidae ) , in the laboratory .
	manualset3
193695	4	415786	7	NULL	NULL	0	NULL	Glossina morsitans ( Diptera : Glossinidae )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Trypanosoma brucei rhodesiense : mechanical transmission by tsetse , Glossina morsitans ( Diptera : Glossinidae ) , in the laboratory .
	manualset3
193696	5	415786	7	NULL	NULL	NULL	NULL	laboratory	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Trypanosoma brucei rhodesiense : mechanical transmission by tsetse , Glossina morsitans ( Diptera : Glossinidae ) , in the laboratory .
	manualset3
193697	1	415787	7	NULL	NULL	0	NULL	marking	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After marking the lesion and injecting a solution into the submucosa , the lesion was separated from the surrounding normal mucosa following complete incision around the lesion using the GSF .
	manualset3
193698	2	415787	7	NULL	NULL	0	NULL	 lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After marking the lesion and injecting a solution into the submucosa , the lesion was separated from the surrounding normal mucosa following complete incision around the lesion using the GSF .
	manualset3
193699	3	415787	7	NULL	NULL	0	NULL	solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After marking the lesion and injecting a solution into the submucosa , the lesion was separated from the surrounding normal mucosa following complete incision around the lesion using the GSF .
	manualset3
193700	4	415787	7	NULL	NULL	0	NULL	submucosa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After marking the lesion and injecting a solution into the submucosa , the lesion was separated from the surrounding normal mucosa following complete incision around the lesion using the GSF .
	manualset3
193701	5	415787	7	NULL	NULL	0	NULL	 lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After marking the lesion and injecting a solution into the submucosa , the lesion was separated from the surrounding normal mucosa following complete incision around the lesion using the GSF .
	manualset3
193702	6	415787	7	NULL	NULL	0	NULL	normal mucosa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After marking the lesion and injecting a solution into the submucosa , the lesion was separated from the surrounding normal mucosa following complete incision around the lesion using the GSF .
	manualset3
193703	7	415787	7	NULL	NULL	0	NULL	complete incision	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After marking the lesion and injecting a solution into the submucosa , the lesion was separated from the surrounding normal mucosa following complete incision around the lesion using the GSF .
	manualset3
193704	8	415787	7	NULL	NULL	0	NULL	lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After marking the lesion and injecting a solution into the submucosa , the lesion was separated from the surrounding normal mucosa following complete incision around the lesion using the GSF .
	manualset3
193705	9	415787	7	NULL	NULL	0	NULL	GSF	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	After marking the lesion and injecting a solution into the submucosa , the lesion was separated from the surrounding normal mucosa following complete incision around the lesion using the GSF .
	manualset3
193706	1	415788	7	NULL	NULL	NULL	NULL	Trypsinization	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Trypsinization of high-density MDCK cells immediately increased phospho-ERK1 / 2 and was followed by a transient increase in cyclin D1 levels .
	manualset3
193707	2	415788	7	NULL	NULL	0	NULL	high-density MDCK cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Trypsinization of high-density MDCK cells immediately increased phospho-ERK1 / 2 and was followed by a transient increase in cyclin D1 levels .
	manualset3
193708	3	415788	7	NULL	NULL	0	NULL	phospho-ERK1 / 2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Trypsinization of high-density MDCK cells immediately increased phospho-ERK1 / 2 and was followed by a transient increase in cyclin D1 levels .
	manualset3
193709	4	415788	7	NULL	NULL	0	NULL	transient increase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Trypsinization of high-density MDCK cells immediately increased phospho-ERK1 / 2 and was followed by a transient increase in cyclin D1 levels .
	manualset3
193710	5	415788	7	NULL	NULL	0	NULL	cyclin D1 levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Trypsinization of high-density MDCK cells immediately increased phospho-ERK1 / 2 and was followed by a transient increase in cyclin D1 levels .
	manualset3
193711	1	415789	7	NULL	NULL	0	NULL	Tryptase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Tryptase purified by this technique had a specific activity with p-tosyl-L-arginine methyl ester of 117 + / - 9 U/mg and had 3.9 + / - 0.3 active sites per molecule of active enzyme ( 134 , 000 m.w. ) as titrated with p-nitrophenyl-p ' - guanidinobenzoate .
	manualset3
193712	2	415789	7	NULL	NULL	0	NULL	technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Tryptase purified by this technique had a specific activity with p-tosyl-L-arginine methyl ester of 117 + / - 9 U/mg and had 3.9 + / - 0.3 active sites per molecule of active enzyme ( 134 , 000 m.w. ) as titrated with p-nitrophenyl-p ' - guanidinobenzoate .
	manualset3
193713	3	415789	7	NULL	NULL	0	NULL	specific activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Tryptase purified by this technique had a specific activity with p-tosyl-L-arginine methyl ester of 117 + / - 9 U/mg and had 3.9 + / - 0.3 active sites per molecule of active enzyme ( 134 , 000 m.w. ) as titrated with p-nitrophenyl-p ' - guanidinobenzoate .
	manualset3
193714	4	415789	7	NULL	NULL	0	NULL	p-tosyl-L-arginine methyl ester 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Tryptase purified by this technique had a specific activity with p-tosyl-L-arginine methyl ester of 117 + / - 9 U/mg and had 3.9 + / - 0.3 active sites per molecule of active enzyme ( 134 , 000 m.w. ) as titrated with p-nitrophenyl-p ' - guanidinobenzoate .
	manualset3
193715	5	415789	7	NULL	NULL	0	NULL	117 + / - 9 U/mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Tryptase purified by this technique had a specific activity with p-tosyl-L-arginine methyl ester of 117 + / - 9 U/mg and had 3.9 + / - 0.3 active sites per molecule of active enzyme ( 134 , 000 m.w. ) as titrated with p-nitrophenyl-p ' - guanidinobenzoate .
	manualset3
193716	6	415789	7	NULL	NULL	0	NULL	3.9 + / - 0.3	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Tryptase purified by this technique had a specific activity with p-tosyl-L-arginine methyl ester of 117 + / - 9 U/mg and had 3.9 + / - 0.3 active sites per molecule of active enzyme ( 134 , 000 m.w. ) as titrated with p-nitrophenyl-p ' - guanidinobenzoate .
	manualset3
193717	7	415789	7	NULL	NULL	0	NULL	active sites per molecule	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Tryptase purified by this technique had a specific activity with p-tosyl-L-arginine methyl ester of 117 + / - 9 U/mg and had 3.9 + / - 0.3 active sites per molecule of active enzyme ( 134 , 000 m.w. ) as titrated with p-nitrophenyl-p ' - guanidinobenzoate .
	manualset3
193718	8	415789	7	NULL	NULL	0	NULL	active enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Tryptase purified by this technique had a specific activity with p-tosyl-L-arginine methyl ester of 117 + / - 9 U/mg and had 3.9 + / - 0.3 active sites per molecule of active enzyme ( 134 , 000 m.w. ) as titrated with p-nitrophenyl-p ' - guanidinobenzoate .
	manualset3
193719	9	415789	7	NULL	NULL	0	NULL	134 , 000 m.w.	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Tryptase purified by this technique had a specific activity with p-tosyl-L-arginine methyl ester of 117 + / - 9 U/mg and had 3.9 + / - 0.3 active sites per molecule of active enzyme ( 134 , 000 m.w. ) as titrated with p-nitrophenyl-p ' - guanidinobenzoate .
	manualset3
193720	10	415789	7	NULL	NULL	0	NULL	p-nitrophenyl-p ' - guanidinobenzoate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Tryptase purified by this technique had a specific activity with p-tosyl-L-arginine methyl ester of 117 + / - 9 U/mg and had 3.9 + / - 0.3 active sites per molecule of active enzyme ( 134 , 000 m.w. ) as titrated with p-nitrophenyl-p ' - guanidinobenzoate .
	manualset3
193721	1	415790	7	NULL	NULL	0	NULL	Tuberculosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Tuberculosis among garment workers in an Arabian developing country : State of Qatar .
	manualset3
193722	2	415790	7	NULL	NULL	0	NULL	garment workers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Tuberculosis among garment workers in an Arabian developing country : State of Qatar .
	manualset3
193723	3	415790	7	NULL	NULL	0	NULL	Arabian developing country	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Tuberculosis among garment workers in an Arabian developing country : State of Qatar .
	manualset3
193724	4	415790	7	NULL	NULL	0	NULL	State of Qatar 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Tuberculosis among garment workers in an Arabian developing country : State of Qatar .
	manualset3
193725	1	415791	7	NULL	NULL	0	NULL	Tuberculosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Tuberculosis complicated with infliximab therapy is one of the most important concerns in Japan .
	manualset3
193726	2	415791	7	NULL	NULL	0	NULL	 infliximab therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Tuberculosis complicated with infliximab therapy is one of the most important concerns in Japan .
	manualset3
193727	3	415791	7	NULL	NULL	0	NULL	 concerns	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Tuberculosis complicated with infliximab therapy is one of the most important concerns in Japan .
	manualset3
193728	4	415791	7	NULL	NULL	0	NULL	Japan	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Tuberculosis complicated with infliximab therapy is one of the most important concerns in Japan .
	manualset3
193729	1	415792	7	NULL	NULL	0	NULL	Tuberculosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Tuberculosis is the world 's leading cause of death due to a single infectious agent , and efforts aimed at its control require a better understanding of host , environmental , and bacterial factors that govern disease outcome .
	manualset3
193730	3	415792	7	NULL	NULL	NULL	NULL	death	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Tuberculosis is the world 's leading cause of death due to a single infectious agent , and efforts aimed at its control require a better understanding of host , environmental , and bacterial factors that govern disease outcome .
	manualset3
193731	2	415792	7	NULL	NULL	NULL	NULL	leading cause	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Tuberculosis is the world 's leading cause of death due to a single infectious agent , and efforts aimed at its control require a better understanding of host , environmental , and bacterial factors that govern disease outcome .
	manualset3
193732	4	415792	7	NULL	NULL	0	NULL	single infectious agent	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Tuberculosis is the world 's leading cause of death due to a single infectious agent , and efforts aimed at its control require a better understanding of host , environmental , and bacterial factors that govern disease outcome .
	manualset3
193733	5	415792	7	NULL	NULL	0	NULL	efforts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Tuberculosis is the world 's leading cause of death due to a single infectious agent , and efforts aimed at its control require a better understanding of host , environmental , and bacterial factors that govern disease outcome .
	manualset3
193734	6	415792	7	NULL	NULL	0	NULL	control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Tuberculosis is the world 's leading cause of death due to a single infectious agent , and efforts aimed at its control require a better understanding of host , environmental , and bacterial factors that govern disease outcome .
	manualset3
193735	7	415792	7	NULL	NULL	0	NULL	understanding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Tuberculosis is the world 's leading cause of death due to a single infectious agent , and efforts aimed at its control require a better understanding of host , environmental , and bacterial factors that govern disease outcome .
	manualset3
193736	8	415792	7	NULL	NULL	0	NULL	host	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Tuberculosis is the world 's leading cause of death due to a single infectious agent , and efforts aimed at its control require a better understanding of host , environmental , and bacterial factors that govern disease outcome .
	manualset3
193737	9	415792	7	NULL	NULL	0	NULL	environmental factors	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Tuberculosis is the world 's leading cause of death due to a single infectious agent , and efforts aimed at its control require a better understanding of host , environmental , and bacterial factors that govern disease outcome .
	manualset3
193738	10	415792	7	NULL	NULL	0	NULL	bacterial factors	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Tuberculosis is the world 's leading cause of death due to a single infectious agent , and efforts aimed at its control require a better understanding of host , environmental , and bacterial factors that govern disease outcome .
	manualset3
193739	11	415792	7	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Tuberculosis is the world 's leading cause of death due to a single infectious agent , and efforts aimed at its control require a better understanding of host , environmental , and bacterial factors that govern disease outcome .
	manualset3
193740	1	415793	7	NULL	NULL	0	NULL	Tuberous sclerosis ( TSC )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Tuberous sclerosis ( TSC ) is an autosomal dominant disorder characterized by a broad phenotypic spectrum that includes seizures , mental retardation , renal dysfunction and dermatological abnormalities .
	manualset3
193741	2	415793	7	NULL	NULL	0	NULL	autosomal dominant disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Tuberous sclerosis ( TSC ) is an autosomal dominant disorder characterized by a broad phenotypic spectrum that includes seizures , mental retardation , renal dysfunction and dermatological abnormalities .
	manualset3
193742	3	415793	7	NULL	NULL	0	NULL	broad phenotypic spectrum	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Tuberous sclerosis ( TSC ) is an autosomal dominant disorder characterized by a broad phenotypic spectrum that includes seizures , mental retardation , renal dysfunction and dermatological abnormalities .
	manualset3
193743	4	415793	7	NULL	NULL	NULL	NULL	seizures	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Tuberous sclerosis ( TSC ) is an autosomal dominant disorder characterized by a broad phenotypic spectrum that includes seizures , mental retardation , renal dysfunction and dermatological abnormalities .
	manualset3
193744	5	415793	7	NULL	NULL	NULL	NULL	mental retardation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Tuberous sclerosis ( TSC ) is an autosomal dominant disorder characterized by a broad phenotypic spectrum that includes seizures , mental retardation , renal dysfunction and dermatological abnormalities .
	manualset3
193745	6	415793	7	NULL	NULL	NULL	NULL	renal dysfunction	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Tuberous sclerosis ( TSC ) is an autosomal dominant disorder characterized by a broad phenotypic spectrum that includes seizures , mental retardation , renal dysfunction and dermatological abnormalities .
	manualset3
193746	7	415793	7	NULL	NULL	NULL	NULL	dermatological abnormalities	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Tuberous sclerosis ( TSC ) is an autosomal dominant disorder characterized by a broad phenotypic spectrum that includes seizures , mental retardation , renal dysfunction and dermatological abnormalities .
	manualset3
193747	1	415794	7	NULL	NULL	0	NULL	Tuberous sclerosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Tuberous sclerosis and multiple intracranial aneurysms : case report .
	manualset3
193748	2	415794	7	NULL	NULL	0	NULL	multiple intracranial aneurysms	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Tuberous sclerosis and multiple intracranial aneurysms : case report .
	manualset3
193749	3	415794	7	NULL	NULL	0	NULL	case report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Tuberous sclerosis and multiple intracranial aneurysms : case report .
	manualset3
193750	1	415795	7	NULL	NULL	0	NULL	Tuftelin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Tuftelin is an acidic protein expressed at very early stages of mouse odontogenesis .
	manualset3
193751	2	415795	7	NULL	NULL	0	NULL	acidic protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Tuftelin is an acidic protein expressed at very early stages of mouse odontogenesis .
	manualset3
193752	3	415795	7	NULL	NULL	0	NULL	early stages	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Tuftelin is an acidic protein expressed at very early stages of mouse odontogenesis .
	manualset3
193753	4	415795	7	NULL	NULL	0	NULL	mouse odontogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Tuftelin is an acidic protein expressed at very early stages of mouse odontogenesis .
	manualset3
193754	1	415796	7	NULL	NULL	0	NULL	Tumor-associated macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor-associated macrophages are a prominent component of ovarian cancer stroma and contribute to tumor progression .
	manualset3
193849	2	415796	7	NULL	NULL	0	NULL	component	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor-associated macrophages are a prominent component of ovarian cancer stroma and contribute to tumor progression .
	manualset3
193850	3	415796	7	NULL	NULL	0	NULL	ovarian cancer stroma	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor-associated macrophages are a prominent component of ovarian cancer stroma and contribute to tumor progression .
	manualset3
193851	4	415796	7	NULL	NULL	0	NULL	tumor progression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor-associated macrophages are a prominent component of ovarian cancer stroma and contribute to tumor progression .
	manualset3
193852	1	415797	7	NULL	NULL	0	NULL	Tumor-bearing mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor-bearing mice infected with Escherichia coli ( E. coli ) intravenously and intraperitoneally showed an apparent delay in the clearance of bacteria compared to the non-tumor-bearing control mice .
	manualset3
193853	2	415797	7	NULL	NULL	0	NULL	Escherichia coli ( E. coli )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor-bearing mice infected with Escherichia coli ( E. coli ) intravenously and intraperitoneally showed an apparent delay in the clearance of bacteria compared to the non-tumor-bearing control mice .
	manualset3
193854	3	415797	7	NULL	NULL	0	NULL	apparent delay	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor-bearing mice infected with Escherichia coli ( E. coli ) intravenously and intraperitoneally showed an apparent delay in the clearance of bacteria compared to the non-tumor-bearing control mice .
	manualset3
193855	4	415797	7	NULL	NULL	0	NULL	clearance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor-bearing mice infected with Escherichia coli ( E. coli ) intravenously and intraperitoneally showed an apparent delay in the clearance of bacteria compared to the non-tumor-bearing control mice .
	manualset3
193856	5	415797	7	NULL	NULL	0	NULL	bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor-bearing mice infected with Escherichia coli ( E. coli ) intravenously and intraperitoneally showed an apparent delay in the clearance of bacteria compared to the non-tumor-bearing control mice .
	manualset3
193857	6	415797	7	NULL	NULL	0	NULL	non-tumor-bearing control mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor-bearing mice infected with Escherichia coli ( E. coli ) intravenously and intraperitoneally showed an apparent delay in the clearance of bacteria compared to the non-tumor-bearing control mice .
	manualset3
193858	1	415798	7	NULL	NULL	0	NULL	Tumor angiogenesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor angiogenesis is the process by which new blood vessels are formed and enhance the oxygenation and growth of tumors .
	manualset3
193859	2	415798	7	NULL	NULL	0	NULL	 process	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor angiogenesis is the process by which new blood vessels are formed and enhance the oxygenation and growth of tumors .
	manualset3
193860	3	415798	7	NULL	NULL	0	NULL	 new blood vessels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor angiogenesis is the process by which new blood vessels are formed and enhance the oxygenation and growth of tumors .
	manualset3
193861	4	415798	7	NULL	NULL	0	NULL	oxygenation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor angiogenesis is the process by which new blood vessels are formed and enhance the oxygenation and growth of tumors .
	manualset3
193862	5	415798	7	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor angiogenesis is the process by which new blood vessels are formed and enhance the oxygenation and growth of tumors .
	manualset3
193863	6	415798	7	NULL	NULL	0	NULL	tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor angiogenesis is the process by which new blood vessels are formed and enhance the oxygenation and growth of tumors .
	manualset3
193864	1	415799	7	NULL	NULL	0	NULL	Tumor cell growth inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor cell growth inhibition and extracellular signal-regulated kinase ( ERK ) phosphorylation by novel K vitamins .
	manualset3
193865	2	415799	7	NULL	NULL	0	NULL	extracellular signal-regulated kinase ( ERK ) phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor cell growth inhibition and extracellular signal-regulated kinase ( ERK ) phosphorylation by novel K vitamins .
	manualset3
193866	3	415799	7	NULL	NULL	0	NULL	novel K vitamins	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor cell growth inhibition and extracellular signal-regulated kinase ( ERK ) phosphorylation by novel K vitamins .
	manualset3
193867	1	415800	7	NULL	NULL	0	NULL	Tumor suppression 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor suppression by pRB has been linked to its ability to repress E2F-responsive promoters such as the E2F-1 promoter .
	manualset3
193868	2	415800	7	NULL	NULL	0	NULL	pRB 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor suppression by pRB has been linked to its ability to repress E2F-responsive promoters such as the E2F-1 promoter .
	manualset3
193869	3	415800	7	NULL	NULL	0	NULL	E2F-responsive promoters	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor suppression by pRB has been linked to its ability to repress E2F-responsive promoters such as the E2F-1 promoter .
	manualset3
193870	4	415800	7	NULL	NULL	0	NULL	E2F-1 promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor suppression by pRB has been linked to its ability to repress E2F-responsive promoters such as the E2F-1 promoter .
	manualset3
193871	1	415801	7	NULL	NULL	0	NULL	Tumor visualization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor visualization was seen to be dose-related .
	manualset3
193872	2	415801	7	NULL	NULL	0	NULL	dose-related 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor visualization was seen to be dose-related .
	manualset3
193873	1	415802	7	NULL	NULL	0	NULL	Tumor 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor was successfully visualized by NIRF and MRI in vivo by intravenously injected PCM-CS .
	manualset3
193874	2	415802	7	NULL	NULL	0	NULL	NIRF	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor was successfully visualized by NIRF and MRI in vivo by intravenously injected PCM-CS .
	manualset3
193875	3	415802	7	NULL	NULL	0	NULL	MRI	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor was successfully visualized by NIRF and MRI in vivo by intravenously injected PCM-CS .
	manualset3
193876	4	415802	7	NULL	NULL	0	NULL	PCM-CS	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor was successfully visualized by NIRF and MRI in vivo by intravenously injected PCM-CS .
	manualset3
193877	1	415803	7	NULL	NULL	0	NULL	Tumors 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumors are dependent on cellular stress responses , in particular the heat shock response , for survival in their hypoxic , acidotic , and nutrient-deprived microenvironments .
	manualset3
193878	2	415803	7	NULL	NULL	0	NULL	cellular stress responses 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumors are dependent on cellular stress responses , in particular the heat shock response , for survival in their hypoxic , acidotic , and nutrient-deprived microenvironments .
	manualset3
193879	3	415803	7	NULL	NULL	0	NULL	heat shock response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumors are dependent on cellular stress responses , in particular the heat shock response , for survival in their hypoxic , acidotic , and nutrient-deprived microenvironments .
	manualset3
193880	4	415803	7	NULL	NULL	0	NULL	survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumors are dependent on cellular stress responses , in particular the heat shock response , for survival in their hypoxic , acidotic , and nutrient-deprived microenvironments .
	manualset3
193881	5	415803	7	NULL	NULL	NULL	NULL	hypoxic microenviroments	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Tumors are dependent on cellular stress responses , in particular the heat shock response , for survival in their hypoxic , acidotic , and nutrient-deprived microenvironments .
	manualset3
193882	6	415803	7	NULL	NULL	0	NULL	acidotic microenvironments	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumors are dependent on cellular stress responses , in particular the heat shock response , for survival in their hypoxic , acidotic , and nutrient-deprived microenvironments .
	manualset3
193883	7	415803	7	NULL	NULL	0	NULL	nutrient-deprived microenvironments	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumors are dependent on cellular stress responses , in particular the heat shock response , for survival in their hypoxic , acidotic , and nutrient-deprived microenvironments .
	manualset3
193884	1	415804	7	NULL	NULL	0	NULL	Tumour type	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumour type , grade , stage and the dimensions of the tumor were recorded .
	manualset3
193885	2	415804	7	NULL	NULL	0	NULL	grade	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumour type , grade , stage and the dimensions of the tumor were recorded .
	manualset3
193886	3	415804	7	NULL	NULL	0	NULL	stage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumour type , grade , stage and the dimensions of the tumor were recorded .
	manualset3
193887	4	415804	7	NULL	NULL	0	NULL	 dimensions 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumour type , grade , stage and the dimensions of the tumor were recorded .
	manualset3
193888	5	415804	7	NULL	NULL	0	NULL	tumor	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumour type , grade , stage and the dimensions of the tumor were recorded .
	manualset3
193889	1	415805	7	NULL	NULL	0	NULL	Turning off 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Turning off a fixation point prior to or coincident with the appearance of a visual target reduces the latency of saccades to that target .
	manualset3
193890	2	415805	7	NULL	NULL	0	NULL	fixation point	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Turning off a fixation point prior to or coincident with the appearance of a visual target reduces the latency of saccades to that target .
	manualset3
193891	3	415805	7	NULL	NULL	0	NULL	appearance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Turning off a fixation point prior to or coincident with the appearance of a visual target reduces the latency of saccades to that target .
	manualset3
193892	4	415805	7	NULL	NULL	NULL	NULL	 visual target	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Turning off a fixation point prior to or coincident with the appearance of a visual target reduces the latency of saccades to that target .
	manualset3
193893	5	415805	7	NULL	NULL	0	NULL	latency	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Turning off a fixation point prior to or coincident with the appearance of a visual target reduces the latency of saccades to that target .
	manualset3
193894	6	415805	7	NULL	NULL	0	NULL	saccades	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Turning off a fixation point prior to or coincident with the appearance of a visual target reduces the latency of saccades to that target .
	manualset3
193895	7	415805	7	NULL	NULL	0	NULL	target	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Turning off a fixation point prior to or coincident with the appearance of a visual target reduces the latency of saccades to that target .
	manualset3
193896	1	415806	7	NULL	NULL	0	NULL	Twelve cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve cases were erroniously diagnosed and confusion with cerebrovascular disease was most common .
	manualset3
193897	2	415806	7	NULL	NULL	0	NULL	cerebrovascular disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve cases were erroniously diagnosed and confusion with cerebrovascular disease was most common .
	manualset3
193898	3	415806	7	NULL	NULL	0	NULL	confusion	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve cases were erroniously diagnosed and confusion with cerebrovascular disease was most common .
	manualset3
193899	1	415807	7	NULL	NULL	0	NULL	Twelve constituents	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve constituents from the volatile oil were identified by method of GC-MS .
	manualset3
193900	2	415807	7	NULL	NULL	0	NULL	volatile oil	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve constituents from the volatile oil were identified by method of GC-MS .
	manualset3
193901	3	415807	7	NULL	NULL	0	NULL	method 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve constituents from the volatile oil were identified by method of GC-MS .
	manualset3
193902	4	415807	7	NULL	NULL	0	NULL	GC-MS	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve constituents from the volatile oil were identified by method of GC-MS .
	manualset3
193903	1	415808	7	NULL	NULL	0	NULL	ondansetron	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	After ondansetron and droperidol , the incidence of severe drowsiness , restlessness , anxiety , or dizziness was 5 % and 28 % , respectively ( P & lt ; 0.01 ) .
	manualset3
193904	2	415808	7	NULL	NULL	0	NULL	 droperidol 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	After ondansetron and droperidol , the incidence of severe drowsiness , restlessness , anxiety , or dizziness was 5 % and 28 % , respectively ( P & lt ; 0.01 ) .
	manualset3
193905	3	415808	7	NULL	NULL	0	NULL	 incidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After ondansetron and droperidol , the incidence of severe drowsiness , restlessness , anxiety , or dizziness was 5 % and 28 % , respectively ( P & lt ; 0.01 ) .
	manualset3
193906	4	415808	7	NULL	NULL	0	NULL	severe drowsiness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After ondansetron and droperidol , the incidence of severe drowsiness , restlessness , anxiety , or dizziness was 5 % and 28 % , respectively ( P & lt ; 0.01 ) .
	manualset3
193907	5	415808	7	NULL	NULL	0	NULL	 restlessness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After ondansetron and droperidol , the incidence of severe drowsiness , restlessness , anxiety , or dizziness was 5 % and 28 % , respectively ( P & lt ; 0.01 ) .
	manualset3
193908	6	415808	7	NULL	NULL	0	NULL	anxiety 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After ondansetron and droperidol , the incidence of severe drowsiness , restlessness , anxiety , or dizziness was 5 % and 28 % , respectively ( P & lt ; 0.01 ) .
	manualset3
193909	7	415808	7	NULL	NULL	0	NULL	 dizziness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After ondansetron and droperidol , the incidence of severe drowsiness , restlessness , anxiety , or dizziness was 5 % and 28 % , respectively ( P & lt ; 0.01 ) .
	manualset3
193910	8	415808	7	NULL	NULL	0	NULL	5 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After ondansetron and droperidol , the incidence of severe drowsiness , restlessness , anxiety , or dizziness was 5 % and 28 % , respectively ( P & lt ; 0.01 ) .
	manualset3
193911	9	415808	7	NULL	NULL	0	NULL	28 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After ondansetron and droperidol , the incidence of severe drowsiness , restlessness , anxiety , or dizziness was 5 % and 28 % , respectively ( P & lt ; 0.01 ) .
	manualset3
193912	10	415808	7	NULL	NULL	0	NULL	P & lt ; 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	After ondansetron and droperidol , the incidence of severe drowsiness , restlessness , anxiety , or dizziness was 5 % and 28 % , respectively ( P & lt ; 0.01 ) .
	manualset3
193913	1	415809	7	NULL	NULL	0	NULL	Twelve patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve patients were evaluable for response and toxicity ( eight with limited disease ) .
	manualset3
193914	2	415809	7	NULL	NULL	0	NULL	response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve patients were evaluable for response and toxicity ( eight with limited disease ) .
	manualset3
193915	3	415809	7	NULL	NULL	0	NULL	toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve patients were evaluable for response and toxicity ( eight with limited disease ) .
	manualset3
193916	4	415809	7	NULL	NULL	0	NULL	eight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve patients were evaluable for response and toxicity ( eight with limited disease ) .
	manualset3
193917	5	415809	7	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve patients were evaluable for response and toxicity ( eight with limited disease ) .
	manualset3
193918	1	415810	7	NULL	NULL	0	NULL	Twelve patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve patients with sinobronchial syndrome who underwent ESS at our department between 1989 and 1993 were enrolled in the study .
	manualset3
193919	2	415810	7	NULL	NULL	0	NULL	sinobronchial syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve patients with sinobronchial syndrome who underwent ESS at our department between 1989 and 1993 were enrolled in the study .
	manualset3
193920	3	415810	7	NULL	NULL	0	NULL	 ESS	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve patients with sinobronchial syndrome who underwent ESS at our department between 1989 and 1993 were enrolled in the study .
	manualset3
193921	4	415810	7	NULL	NULL	0	NULL	department	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve patients with sinobronchial syndrome who underwent ESS at our department between 1989 and 1993 were enrolled in the study .
	manualset3
193922	5	415810	7	NULL	NULL	0	NULL	1989	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve patients with sinobronchial syndrome who underwent ESS at our department between 1989 and 1993 were enrolled in the study .
	manualset3
193923	6	415810	7	NULL	NULL	0	NULL	1993	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve patients with sinobronchial syndrome who underwent ESS at our department between 1989 and 1993 were enrolled in the study .
	manualset3
193924	7	415810	7	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve patients with sinobronchial syndrome who underwent ESS at our department between 1989 and 1993 were enrolled in the study .
	manualset3
193925	1	415811	7	NULL	NULL	0	NULL	Twenty-eight 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-eight Angus ( 289 + / - 3.8 kg ) steers were used in a completely randomized design to evaluate the effect of isocaloric supplementation of 2 different energy sources to steers rotationally grazing tall fescue pastures for 197 d in comparison to positive and negative controls .
	manualset3
193926	2	415811	7	NULL	NULL	0	NULL	Angus steers	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-eight Angus ( 289 + / - 3.8 kg ) steers were used in a completely randomized design to evaluate the effect of isocaloric supplementation of 2 different energy sources to steers rotationally grazing tall fescue pastures for 197 d in comparison to positive and negative controls .
	manualset3
193927	3	415811	7	NULL	NULL	0	NULL	289 + / - 3.8 kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-eight Angus ( 289 + / - 3.8 kg ) steers were used in a completely randomized design to evaluate the effect of isocaloric supplementation of 2 different energy sources to steers rotationally grazing tall fescue pastures for 197 d in comparison to positive and negative controls .
	manualset3
193928	4	415811	7	NULL	NULL	0	NULL	completely randomized design	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-eight Angus ( 289 + / - 3.8 kg ) steers were used in a completely randomized design to evaluate the effect of isocaloric supplementation of 2 different energy sources to steers rotationally grazing tall fescue pastures for 197 d in comparison to positive and negative controls .
	manualset3
193929	5	415811	7	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-eight Angus ( 289 + / - 3.8 kg ) steers were used in a completely randomized design to evaluate the effect of isocaloric supplementation of 2 different energy sources to steers rotationally grazing tall fescue pastures for 197 d in comparison to positive and negative controls .
	manualset3
193930	6	415811	7	NULL	NULL	0	NULL	isocaloric supplementation	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-eight Angus ( 289 + / - 3.8 kg ) steers were used in a completely randomized design to evaluate the effect of isocaloric supplementation of 2 different energy sources to steers rotationally grazing tall fescue pastures for 197 d in comparison to positive and negative controls .
	manualset3
193931	7	415811	7	NULL	NULL	NULL	NULL	2 different energy sources	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Twenty-eight Angus ( 289 + / - 3.8 kg ) steers were used in a completely randomized design to evaluate the effect of isocaloric supplementation of 2 different energy sources to steers rotationally grazing tall fescue pastures for 197 d in comparison to positive and negative controls .
	manualset3
193932	8	415811	7	NULL	NULL	0	NULL	steers 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-eight Angus ( 289 + / - 3.8 kg ) steers were used in a completely randomized design to evaluate the effect of isocaloric supplementation of 2 different energy sources to steers rotationally grazing tall fescue pastures for 197 d in comparison to positive and negative controls .
	manualset3
193933	9	415811	7	NULL	NULL	NULL	NULL	rotationally grazing tall fescue pastures	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Twenty-eight Angus ( 289 + / - 3.8 kg ) steers were used in a completely randomized design to evaluate the effect of isocaloric supplementation of 2 different energy sources to steers rotationally grazing tall fescue pastures for 197 d in comparison to positive and negative controls .
	manualset3
193934	10	415811	7	NULL	NULL	NULL	NULL	 197 d	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Twenty-eight Angus ( 289 + / - 3.8 kg ) steers were used in a completely randomized design to evaluate the effect of isocaloric supplementation of 2 different energy sources to steers rotationally grazing tall fescue pastures for 197 d in comparison to positive and negative controls .
	manualset3
193935	11	415811	7	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-eight Angus ( 289 + / - 3.8 kg ) steers were used in a completely randomized design to evaluate the effect of isocaloric supplementation of 2 different energy sources to steers rotationally grazing tall fescue pastures for 197 d in comparison to positive and negative controls .
	manualset3
193936	12	415811	7	NULL	NULL	0	NULL	positive controls	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-eight Angus ( 289 + / - 3.8 kg ) steers were used in a completely randomized design to evaluate the effect of isocaloric supplementation of 2 different energy sources to steers rotationally grazing tall fescue pastures for 197 d in comparison to positive and negative controls .
	manualset3
193937	13	415811	7	NULL	NULL	0	NULL	negative controls	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-eight Angus ( 289 + / - 3.8 kg ) steers were used in a completely randomized design to evaluate the effect of isocaloric supplementation of 2 different energy sources to steers rotationally grazing tall fescue pastures for 197 d in comparison to positive and negative controls .
	manualset3
193938	1	415812	7	NULL	NULL	0	NULL	Twenty-five men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-five men with testicular germ cell tumors were compared by developmental history and past and present psychologic adjustment to 25 men with acute leukemia .
	manualset3
193939	2	415812	7	NULL	NULL	0	NULL	testicular germ cell tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-five men with testicular germ cell tumors were compared by developmental history and past and present psychologic adjustment to 25 men with acute leukemia .
	manualset3
193940	3	415812	7	NULL	NULL	NULL	NULL	developmental history	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Twenty-five men with testicular germ cell tumors were compared by developmental history and past and present psychologic adjustment to 25 men with acute leukemia .
	manualset3
193941	4	415812	7	NULL	NULL	0	NULL	psychologic adjustment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-five men with testicular germ cell tumors were compared by developmental history and past and present psychologic adjustment to 25 men with acute leukemia .
	manualset3
193942	5	415812	7	NULL	NULL	0	NULL	 25 men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-five men with testicular germ cell tumors were compared by developmental history and past and present psychologic adjustment to 25 men with acute leukemia .
	manualset3
193943	6	415812	7	NULL	NULL	0	NULL	acute leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-five men with testicular germ cell tumors were compared by developmental history and past and present psychologic adjustment to 25 men with acute leukemia .
	manualset3
193944	1	415813	7	NULL	NULL	0	NULL	Twenty-five patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-five patients had a normal prolactin level ( less than or equal to 30 ng/ml ) during the early postoperative period ( less than or equal to 3 months ) and 15 patients had persistent disease ( prolactin greater than 30 ng/ml ) .
	manualset3
193945	2	415813	7	NULL	NULL	0	NULL	normal prolactin level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-five patients had a normal prolactin level ( less than or equal to 30 ng/ml ) during the early postoperative period ( less than or equal to 3 months ) and 15 patients had persistent disease ( prolactin greater than 30 ng/ml ) .
	manualset3
193946	3	415813	7	NULL	NULL	0	NULL	less than 30 ng/ml	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-five patients had a normal prolactin level ( less than or equal to 30 ng/ml ) during the early postoperative period ( less than or equal to 3 months ) and 15 patients had persistent disease ( prolactin greater than 30 ng/ml ) .
	manualset3
193947	4	415813	7	NULL	NULL	0	NULL	equal to 30 ng/ml 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-five patients had a normal prolactin level ( less than or equal to 30 ng/ml ) during the early postoperative period ( less than or equal to 3 months ) and 15 patients had persistent disease ( prolactin greater than 30 ng/ml ) .
	manualset3
193948	5	415813	7	NULL	NULL	0	NULL	early postoperative period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-five patients had a normal prolactin level ( less than or equal to 30 ng/ml ) during the early postoperative period ( less than or equal to 3 months ) and 15 patients had persistent disease ( prolactin greater than 30 ng/ml ) .
	manualset3
193949	6	415813	7	NULL	NULL	0	NULL	less than 3 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-five patients had a normal prolactin level ( less than or equal to 30 ng/ml ) during the early postoperative period ( less than or equal to 3 months ) and 15 patients had persistent disease ( prolactin greater than 30 ng/ml ) .
	manualset3
193950	7	415813	7	NULL	NULL	0	NULL	equal to 3 months 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-five patients had a normal prolactin level ( less than or equal to 30 ng/ml ) during the early postoperative period ( less than or equal to 3 months ) and 15 patients had persistent disease ( prolactin greater than 30 ng/ml ) .
	manualset3
193951	8	415813	7	NULL	NULL	0	NULL	15 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-five patients had a normal prolactin level ( less than or equal to 30 ng/ml ) during the early postoperative period ( less than or equal to 3 months ) and 15 patients had persistent disease ( prolactin greater than 30 ng/ml ) .
	manualset3
193952	9	415813	7	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-five patients had a normal prolactin level ( less than or equal to 30 ng/ml ) during the early postoperative period ( less than or equal to 3 months ) and 15 patients had persistent disease ( prolactin greater than 30 ng/ml ) .
	manualset3
193953	10	415813	7	NULL	NULL	0	NULL	prolactin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-five patients had a normal prolactin level ( less than or equal to 30 ng/ml ) during the early postoperative period ( less than or equal to 3 months ) and 15 patients had persistent disease ( prolactin greater than 30 ng/ml ) .
	manualset3
193954	11	415813	7	NULL	NULL	0	NULL	30 ng/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-five patients had a normal prolactin level ( less than or equal to 30 ng/ml ) during the early postoperative period ( less than or equal to 3 months ) and 15 patients had persistent disease ( prolactin greater than 30 ng/ml ) .
	manualset3
193955	1	415814	7	NULL	NULL	0	NULL	Twenty-five patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-five patients had not been treated with HU .
	manualset3
193956	2	415814	7	NULL	NULL	0	NULL	HU	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-five patients had not been treated with HU .
	manualset3
193957	1	415815	7	NULL	NULL	0	NULL	Twenty-four-hour	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-four-hour patterns in human performance , subjective and physiological variables and differences between morning and evening active subjects .
	manualset3
193958	2	415815	7	NULL	NULL	0	NULL	human performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-four-hour patterns in human performance , subjective and physiological variables and differences between morning and evening active subjects .
	manualset3
193959	3	415815	7	NULL	NULL	0	NULL	subjective variables	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-four-hour patterns in human performance , subjective and physiological variables and differences between morning and evening active subjects .
	manualset3
193960	4	415815	7	NULL	NULL	0	NULL	physiological variables	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-four-hour patterns in human performance , subjective and physiological variables and differences between morning and evening active subjects .
	manualset3
193961	5	415815	7	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-four-hour patterns in human performance , subjective and physiological variables and differences between morning and evening active subjects .
	manualset3
193962	6	415815	7	NULL	NULL	NULL	NULL	morning active subjects	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Twenty-four-hour patterns in human performance , subjective and physiological variables and differences between morning and evening active subjects .
	manualset3
193963	7	415815	7	NULL	NULL	NULL	NULL	evening active subjects	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Twenty-four-hour patterns in human performance , subjective and physiological variables and differences between morning and evening active subjects .
	manualset3
193965	1	415816	7	NULL	NULL	0	NULL	Twenty-four male	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-four male spontaneously hypertensive rats ( SHR ) , all 7 weeks of age , were assigned randomly to four groups : ( 1 ) control , ( 2 ) cocaine , ( 3 ) nandrolone , and ( 4 ) cocaine plus nandrolone .
	manualset3
193966	2	415816	7	NULL	NULL	0	NULL	spontaneously hypertensive rats ( SHR )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-four male spontaneously hypertensive rats ( SHR ) , all 7 weeks of age , were assigned randomly to four groups : ( 1 ) control , ( 2 ) cocaine , ( 3 ) nandrolone , and ( 4 ) cocaine plus nandrolone .
	manualset3
193967	3	415816	7	NULL	NULL	0	NULL	7 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-four male spontaneously hypertensive rats ( SHR ) , all 7 weeks of age , were assigned randomly to four groups : ( 1 ) control , ( 2 ) cocaine , ( 3 ) nandrolone , and ( 4 ) cocaine plus nandrolone .
	manualset3
193968	4	415816	7	NULL	NULL	0	NULL	age	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-four male spontaneously hypertensive rats ( SHR ) , all 7 weeks of age , were assigned randomly to four groups : ( 1 ) control , ( 2 ) cocaine , ( 3 ) nandrolone , and ( 4 ) cocaine plus nandrolone .
	manualset3
193969	5	415816	7	NULL	NULL	0	NULL	four groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-four male spontaneously hypertensive rats ( SHR ) , all 7 weeks of age , were assigned randomly to four groups : ( 1 ) control , ( 2 ) cocaine , ( 3 ) nandrolone , and ( 4 ) cocaine plus nandrolone .
	manualset3
194019	6	415816	7	NULL	NULL	0	NULL	 control 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-four male spontaneously hypertensive rats ( SHR ) , all 7 weeks of age , were assigned randomly to four groups : ( 1 ) control , ( 2 ) cocaine , ( 3 ) nandrolone , and ( 4 ) cocaine plus nandrolone .
	manualset3
194020	7	415816	7	NULL	NULL	NULL	NULL	 cocaine	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Twenty-four male spontaneously hypertensive rats ( SHR ) , all 7 weeks of age , were assigned randomly to four groups : ( 1 ) control , ( 2 ) cocaine , ( 3 ) nandrolone , and ( 4 ) cocaine plus nandrolone .
	manualset3
194021	8	415816	7	NULL	NULL	0	NULL	nandrolone	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-four male spontaneously hypertensive rats ( SHR ) , all 7 weeks of age , were assigned randomly to four groups : ( 1 ) control , ( 2 ) cocaine , ( 3 ) nandrolone , and ( 4 ) cocaine plus nandrolone .
	manualset3
194022	9	415816	7	NULL	NULL	0	NULL	cocaine plus nandrolone	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-four male spontaneously hypertensive rats ( SHR ) , all 7 weeks of age , were assigned randomly to four groups : ( 1 ) control , ( 2 ) cocaine , ( 3 ) nandrolone , and ( 4 ) cocaine plus nandrolone .
	manualset3
194023	1	415817	7	NULL	NULL	0	NULL	Twenty-four methadone maintenance patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-four methadone maintenance patients were assigned to ( 1 ) decreasing dose ( N = 12 ) or ( 2 ) continued methadone maintenance ( N = 12 ) , matching for dose , initial complaint levels , and counselor .
	manualset3
194024	2	415817	7	NULL	NULL	0	NULL	decreasing dose ( N = 12 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-four methadone maintenance patients were assigned to ( 1 ) decreasing dose ( N = 12 ) or ( 2 ) continued methadone maintenance ( N = 12 ) , matching for dose , initial complaint levels , and counselor .
	manualset3
194025	3	415817	7	NULL	NULL	0	NULL	continued methadone maintenance ( N = 12 )	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-four methadone maintenance patients were assigned to ( 1 ) decreasing dose ( N = 12 ) or ( 2 ) continued methadone maintenance ( N = 12 ) , matching for dose , initial complaint levels , and counselor .
	manualset3
194026	4	415817	7	NULL	NULL	0	NULL	dose 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-four methadone maintenance patients were assigned to ( 1 ) decreasing dose ( N = 12 ) or ( 2 ) continued methadone maintenance ( N = 12 ) , matching for dose , initial complaint levels , and counselor .
	manualset3
194027	5	415817	7	NULL	NULL	0	NULL	initial complaint levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-four methadone maintenance patients were assigned to ( 1 ) decreasing dose ( N = 12 ) or ( 2 ) continued methadone maintenance ( N = 12 ) , matching for dose , initial complaint levels , and counselor .
	manualset3
194028	6	415817	7	NULL	NULL	0	NULL	counselor	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-four methadone maintenance patients were assigned to ( 1 ) decreasing dose ( N = 12 ) or ( 2 ) continued methadone maintenance ( N = 12 ) , matching for dose , initial complaint levels , and counselor .
	manualset3
194029	1	415818	7	NULL	NULL	0	NULL	Twenty-four strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-four strains associated with HeLa cells ( A phenotype ) and 21 elongated CHO ( E phenotype ) .
	manualset3
194030	2	415818	7	NULL	NULL	0	NULL	HeLa cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-four strains associated with HeLa cells ( A phenotype ) and 21 elongated CHO ( E phenotype ) .
	manualset3
194031	3	415818	7	NULL	NULL	0	NULL	A phenotype	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-four strains associated with HeLa cells ( A phenotype ) and 21 elongated CHO ( E phenotype ) .
	manualset3
194032	4	415818	7	NULL	NULL	0	NULL	21 elongated CHO	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-four strains associated with HeLa cells ( A phenotype ) and 21 elongated CHO ( E phenotype ) .
	manualset3
194034	5	415818	7	NULL	NULL	0	NULL	E phenotype	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-four strains associated with HeLa cells ( A phenotype ) and 21 elongated CHO ( E phenotype ) .
	manualset3
194039	1	415819	7	NULL	NULL	0	NULL	Twenty-one patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-one patients ( 30 % ) had evidence of CNS lupus .
	manualset3
194040	2	415819	7	NULL	NULL	0	NULL	30 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-one patients ( 30 % ) had evidence of CNS lupus .
	manualset3
194042	3	415819	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-one patients ( 30 % ) had evidence of CNS lupus .
	manualset3
194043	4	415819	7	NULL	NULL	0	NULL	CNS lupus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-one patients ( 30 % ) had evidence of CNS lupus .
	manualset3
194045	1	415820	7	NULL	NULL	0	NULL	vitamin B6-uptake	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After optimizing the vitamin B6-uptake by means of vitamin administration the differences disappear .
	manualset3
194047	2	415820	7	NULL	NULL	0	NULL	vitamin administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After optimizing the vitamin B6-uptake by means of vitamin administration the differences disappear .
	manualset3
194049	3	415820	7	NULL	NULL	0	NULL	 differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	After optimizing the vitamin B6-uptake by means of vitamin administration the differences disappear .
	manualset3
194057	1	415821	7	NULL	NULL	0	NULL	Twenty-one patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-one patients with serum monoclonal gammopathy but lacking acceptable morphological evidence of myelomatosis were studied with reference to the degree , if any , of monoclonal plasma cell expansion in aspirated marrow samples , enriched for plasma cells and analyzed with respect to light chain distribution .
	manualset3
194059	2	415821	7	NULL	NULL	0	NULL	serum monoclonal gammopathy 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-one patients with serum monoclonal gammopathy but lacking acceptable morphological evidence of myelomatosis were studied with reference to the degree , if any , of monoclonal plasma cell expansion in aspirated marrow samples , enriched for plasma cells and analyzed with respect to light chain distribution .
	manualset3
194060	3	415821	7	NULL	NULL	0	NULL	morphological evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-one patients with serum monoclonal gammopathy but lacking acceptable morphological evidence of myelomatosis were studied with reference to the degree , if any , of monoclonal plasma cell expansion in aspirated marrow samples , enriched for plasma cells and analyzed with respect to light chain distribution .
	manualset3
194062	4	415821	7	NULL	NULL	0	NULL	myelomatosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-one patients with serum monoclonal gammopathy but lacking acceptable morphological evidence of myelomatosis were studied with reference to the degree , if any , of monoclonal plasma cell expansion in aspirated marrow samples , enriched for plasma cells and analyzed with respect to light chain distribution .
	manualset3
194064	5	415821	7	NULL	NULL	0	NULL	reference	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-one patients with serum monoclonal gammopathy but lacking acceptable morphological evidence of myelomatosis were studied with reference to the degree , if any , of monoclonal plasma cell expansion in aspirated marrow samples , enriched for plasma cells and analyzed with respect to light chain distribution .
	manualset3
194068	6	415821	7	NULL	NULL	0	NULL	degree	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-one patients with serum monoclonal gammopathy but lacking acceptable morphological evidence of myelomatosis were studied with reference to the degree , if any , of monoclonal plasma cell expansion in aspirated marrow samples , enriched for plasma cells and analyzed with respect to light chain distribution .
	manualset3
194070	7	415821	7	NULL	NULL	NULL	NULL	monoclonal plasma cell expansion	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Twenty-one patients with serum monoclonal gammopathy but lacking acceptable morphological evidence of myelomatosis were studied with reference to the degree , if any , of monoclonal plasma cell expansion in aspirated marrow samples , enriched for plasma cells and analyzed with respect to light chain distribution .
	manualset3
194071	8	415821	7	NULL	NULL	0	NULL	aspirated marrow samples	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-one patients with serum monoclonal gammopathy but lacking acceptable morphological evidence of myelomatosis were studied with reference to the degree , if any , of monoclonal plasma cell expansion in aspirated marrow samples , enriched for plasma cells and analyzed with respect to light chain distribution .
	manualset3
194072	9	415821	7	NULL	NULL	0	NULL	plasma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-one patients with serum monoclonal gammopathy but lacking acceptable morphological evidence of myelomatosis were studied with reference to the degree , if any , of monoclonal plasma cell expansion in aspirated marrow samples , enriched for plasma cells and analyzed with respect to light chain distribution .
	manualset3
194073	10	415821	7	NULL	NULL	0	NULL	light chain distribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-one patients with serum monoclonal gammopathy but lacking acceptable morphological evidence of myelomatosis were studied with reference to the degree , if any , of monoclonal plasma cell expansion in aspirated marrow samples , enriched for plasma cells and analyzed with respect to light chain distribution .
	manualset3
194074	1	415822	7	NULL	NULL	0	NULL	Twenty-one probable new genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-one probable new genes with more than 50 amino acids have been obtained excluding 13 ORFs which are similar to the genes of NCBI and relative articles .
	manualset3
194075	2	415822	7	NULL	NULL	0	NULL	50 amino acids	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-one probable new genes with more than 50 amino acids have been obtained excluding 13 ORFs which are similar to the genes of NCBI and relative articles .
	manualset3
194076	3	415822	7	NULL	NULL	0	NULL	13 ORFs 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-one probable new genes with more than 50 amino acids have been obtained excluding 13 ORFs which are similar to the genes of NCBI and relative articles .
	manualset3
194077	4	415822	7	NULL	NULL	0	NULL	genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-one probable new genes with more than 50 amino acids have been obtained excluding 13 ORFs which are similar to the genes of NCBI and relative articles .
	manualset3
194078	5	415822	7	NULL	NULL	0	NULL	NCBI	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-one probable new genes with more than 50 amino acids have been obtained excluding 13 ORFs which are similar to the genes of NCBI and relative articles .
	manualset3
194079	6	415822	7	NULL	NULL	0	NULL	articles	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-one probable new genes with more than 50 amino acids have been obtained excluding 13 ORFs which are similar to the genes of NCBI and relative articles .
	manualset3
194080	1	415823	7	NULL	NULL	0	NULL	orally dosing mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	After orally dosing mice with 1-aminocyclopropanecarboxylic acid ( 300 mg/kg ) , 46 and 10 % of the dose was excreted unchanged in the 0-24 h and 24-48 h urines , respectively .
	manualset3
194081	2	415823	7	NULL	NULL	0	NULL	1-aminocyclopropanecarboxylic acid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After orally dosing mice with 1-aminocyclopropanecarboxylic acid ( 300 mg/kg ) , 46 and 10 % of the dose was excreted unchanged in the 0-24 h and 24-48 h urines , respectively .
	manualset3
194082	3	415823	7	NULL	NULL	0	NULL	 300 mg/kg 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After orally dosing mice with 1-aminocyclopropanecarboxylic acid ( 300 mg/kg ) , 46 and 10 % of the dose was excreted unchanged in the 0-24 h and 24-48 h urines , respectively .
	manualset3
194083	4	415823	7	NULL	NULL	0	NULL	46%	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After orally dosing mice with 1-aminocyclopropanecarboxylic acid ( 300 mg/kg ) , 46 and 10 % of the dose was excreted unchanged in the 0-24 h and 24-48 h urines , respectively .
	manualset3
194084	5	415823	7	NULL	NULL	0	NULL	10%	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After orally dosing mice with 1-aminocyclopropanecarboxylic acid ( 300 mg/kg ) , 46 and 10 % of the dose was excreted unchanged in the 0-24 h and 24-48 h urines , respectively .
	manualset3
194085	6	415823	7	NULL	NULL	0	NULL	dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After orally dosing mice with 1-aminocyclopropanecarboxylic acid ( 300 mg/kg ) , 46 and 10 % of the dose was excreted unchanged in the 0-24 h and 24-48 h urines , respectively .
	manualset3
194086	7	415823	7	NULL	NULL	0	NULL	0-24 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After orally dosing mice with 1-aminocyclopropanecarboxylic acid ( 300 mg/kg ) , 46 and 10 % of the dose was excreted unchanged in the 0-24 h and 24-48 h urines , respectively .
	manualset3
194087	8	415823	7	NULL	NULL	0	NULL	24-48 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After orally dosing mice with 1-aminocyclopropanecarboxylic acid ( 300 mg/kg ) , 46 and 10 % of the dose was excreted unchanged in the 0-24 h and 24-48 h urines , respectively .
	manualset3
194088	9	415823	7	NULL	NULL	0	NULL	urines	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After orally dosing mice with 1-aminocyclopropanecarboxylic acid ( 300 mg/kg ) , 46 and 10 % of the dose was excreted unchanged in the 0-24 h and 24-48 h urines , respectively .
	manualset3
194089	1	415824	7	NULL	NULL	0	NULL	Twenty-six novel single nucleotide polymorphisms	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-six novel single nucleotide polymorphisms and their frequencies of the NR1I3 ( CAR ) gene in a Japanese population .
	manualset3
194090	2	415824	7	NULL	NULL	0	NULL	frequencies	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-six novel single nucleotide polymorphisms and their frequencies of the NR1I3 ( CAR ) gene in a Japanese population .
	manualset3
194091	3	415824	7	NULL	NULL	0	NULL	NR1I3 ( CAR ) gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-six novel single nucleotide polymorphisms and their frequencies of the NR1I3 ( CAR ) gene in a Japanese population .
	manualset3
194092	4	415824	7	NULL	NULL	0	NULL	Japanese population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-six novel single nucleotide polymorphisms and their frequencies of the NR1I3 ( CAR ) gene in a Japanese population .
	manualset3
194093	1	415825	7	NULL	NULL	0	NULL	Twenty-six patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-six patients with ConHD and 22 healthy participants categorized heart-related ( heart rate ) or neutral sensations ( constant vibration ) as either heart or neutral .
	manualset3
194094	2	415825	7	NULL	NULL	0	NULL	ConHD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-six patients with ConHD and 22 healthy participants categorized heart-related ( heart rate ) or neutral sensations ( constant vibration ) as either heart or neutral .
	manualset3
194095	3	415825	7	NULL	NULL	0	NULL	22 healthy participants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-six patients with ConHD and 22 healthy participants categorized heart-related ( heart rate ) or neutral sensations ( constant vibration ) as either heart or neutral .
	manualset3
194096	4	415825	7	NULL	NULL	0	NULL	heart-related ( heart rate )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-six patients with ConHD and 22 healthy participants categorized heart-related ( heart rate ) or neutral sensations ( constant vibration ) as either heart or neutral .
	manualset3
194097	5	415825	7	NULL	NULL	0	NULL	neutral sensations ( constant vibration )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-six patients with ConHD and 22 healthy participants categorized heart-related ( heart rate ) or neutral sensations ( constant vibration ) as either heart or neutral .
	manualset3
194098	6	415825	7	NULL	NULL	0	NULL	heart 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-six patients with ConHD and 22 healthy participants categorized heart-related ( heart rate ) or neutral sensations ( constant vibration ) as either heart or neutral .
	manualset3
194099	7	415825	7	NULL	NULL	0	NULL	neutral	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-six patients with ConHD and 22 healthy participants categorized heart-related ( heart rate ) or neutral sensations ( constant vibration ) as either heart or neutral .
	manualset3
194100	1	415826	7	NULL	NULL	0	NULL	Twenty-three patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-three patients , who were treated from January 1987 to August 1989 , had spinal fluid drainage ( group B ) ; 12 patients in this group also received naloxone as an intravenous drip at 1 microgram/kg/hr for 48 hours after surgery .
	manualset3
194101	2	415826	7	NULL	NULL	NULL	NULL	January 1987	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Twenty-three patients , who were treated from January 1987 to August 1989 , had spinal fluid drainage ( group B ) ; 12 patients in this group also received naloxone as an intravenous drip at 1 microgram/kg/hr for 48 hours after surgery .
	manualset3
194102	3	415826	7	NULL	NULL	0	NULL	August 1989	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-three patients , who were treated from January 1987 to August 1989 , had spinal fluid drainage ( group B ) ; 12 patients in this group also received naloxone as an intravenous drip at 1 microgram/kg/hr for 48 hours after surgery .
	manualset3
194103	4	415826	7	NULL	NULL	0	NULL	spinal fluid drainage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-three patients , who were treated from January 1987 to August 1989 , had spinal fluid drainage ( group B ) ; 12 patients in this group also received naloxone as an intravenous drip at 1 microgram/kg/hr for 48 hours after surgery .
	manualset3
194104	5	415826	7	NULL	NULL	0	NULL	group B	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-three patients , who were treated from January 1987 to August 1989 , had spinal fluid drainage ( group B ) ; 12 patients in this group also received naloxone as an intravenous drip at 1 microgram/kg/hr for 48 hours after surgery .
	manualset3
194105	6	415826	7	NULL	NULL	0	NULL	12 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-three patients , who were treated from January 1987 to August 1989 , had spinal fluid drainage ( group B ) ; 12 patients in this group also received naloxone as an intravenous drip at 1 microgram/kg/hr for 48 hours after surgery .
	manualset3
194106	7	415826	7	NULL	NULL	0	NULL	group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-three patients , who were treated from January 1987 to August 1989 , had spinal fluid drainage ( group B ) ; 12 patients in this group also received naloxone as an intravenous drip at 1 microgram/kg/hr for 48 hours after surgery .
	manualset3
194107	8	415826	7	NULL	NULL	0	NULL	naloxone 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-three patients , who were treated from January 1987 to August 1989 , had spinal fluid drainage ( group B ) ; 12 patients in this group also received naloxone as an intravenous drip at 1 microgram/kg/hr for 48 hours after surgery .
	manualset3
194108	9	415826	7	NULL	NULL	0	NULL	intravenous drip	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-three patients , who were treated from January 1987 to August 1989 , had spinal fluid drainage ( group B ) ; 12 patients in this group also received naloxone as an intravenous drip at 1 microgram/kg/hr for 48 hours after surgery .
	manualset3
194109	10	415826	7	NULL	NULL	0	NULL	1 microgram/kg/hr	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-three patients , who were treated from January 1987 to August 1989 , had spinal fluid drainage ( group B ) ; 12 patients in this group also received naloxone as an intravenous drip at 1 microgram/kg/hr for 48 hours after surgery .
	manualset3
194110	11	415826	7	NULL	NULL	0	NULL	48 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-three patients , who were treated from January 1987 to August 1989 , had spinal fluid drainage ( group B ) ; 12 patients in this group also received naloxone as an intravenous drip at 1 microgram/kg/hr for 48 hours after surgery .
	manualset3
194111	12	415826	7	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-three patients , who were treated from January 1987 to August 1989 , had spinal fluid drainage ( group B ) ; 12 patients in this group also received naloxone as an intravenous drip at 1 microgram/kg/hr for 48 hours after surgery .
	manualset3
194112	1	415827	7	NULL	NULL	0	NULL	Twenty-three percent ( seven ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-three percent ( seven ) of the patients stopped taking modafinil during the study owing to one of the following : decreased sleep time ( four ) , decreased appetite ( one ) , hyperactivity , and irritability ( two ) .
	manualset3
194113	2	415827	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-three percent ( seven ) of the patients stopped taking modafinil during the study owing to one of the following : decreased sleep time ( four ) , decreased appetite ( one ) , hyperactivity , and irritability ( two ) .
	manualset3
194114	3	415827	7	NULL	NULL	0	NULL	modafinil	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-three percent ( seven ) of the patients stopped taking modafinil during the study owing to one of the following : decreased sleep time ( four ) , decreased appetite ( one ) , hyperactivity , and irritability ( two ) .
	manualset3
194115	4	415827	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-three percent ( seven ) of the patients stopped taking modafinil during the study owing to one of the following : decreased sleep time ( four ) , decreased appetite ( one ) , hyperactivity , and irritability ( two ) .
	manualset3
194116	5	415827	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-three percent ( seven ) of the patients stopped taking modafinil during the study owing to one of the following : decreased sleep time ( four ) , decreased appetite ( one ) , hyperactivity , and irritability ( two ) .
	manualset3
194117	6	415827	7	NULL	NULL	0	NULL	decreased sleep time ( four )	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-three percent ( seven ) of the patients stopped taking modafinil during the study owing to one of the following : decreased sleep time ( four ) , decreased appetite ( one ) , hyperactivity , and irritability ( two ) .
	manualset3
194118	7	415827	7	NULL	NULL	0	NULL	decreased appetite ( one )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-three percent ( seven ) of the patients stopped taking modafinil during the study owing to one of the following : decreased sleep time ( four ) , decreased appetite ( one ) , hyperactivity , and irritability ( two ) .
	manualset3
194119	8	415827	7	NULL	NULL	0	NULL	hyperactivity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-three percent ( seven ) of the patients stopped taking modafinil during the study owing to one of the following : decreased sleep time ( four ) , decreased appetite ( one ) , hyperactivity , and irritability ( two ) .
	manualset3
194120	9	415827	7	NULL	NULL	0	NULL	irritability ( two )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-three percent ( seven ) of the patients stopped taking modafinil during the study owing to one of the following : decreased sleep time ( four ) , decreased appetite ( one ) , hyperactivity , and irritability ( two ) .
	manualset3
194121	10	415827	7	NULL	NULL	0	NULL	following	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-three percent ( seven ) of the patients stopped taking modafinil during the study owing to one of the following : decreased sleep time ( four ) , decreased appetite ( one ) , hyperactivity , and irritability ( two ) .
	manualset3
194122	1	415828	7	NULL	NULL	0	NULL	Twenty-two ( 81 % )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two ( 81 % ) of the patients ovulated according to basal body temperature and progesterone values , and 20 ( 74 % ) conceived during one to four treatment cycles .
	manualset3
194123	2	415828	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two ( 81 % ) of the patients ovulated according to basal body temperature and progesterone values , and 20 ( 74 % ) conceived during one to four treatment cycles .
	manualset3
194124	3	415828	7	NULL	NULL	0	NULL	basal body temperature	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two ( 81 % ) of the patients ovulated according to basal body temperature and progesterone values , and 20 ( 74 % ) conceived during one to four treatment cycles .
	manualset3
194125	4	415828	7	NULL	NULL	0	NULL	progesterone values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two ( 81 % ) of the patients ovulated according to basal body temperature and progesterone values , and 20 ( 74 % ) conceived during one to four treatment cycles .
	manualset3
194126	5	415828	7	NULL	NULL	0	NULL	20 ( 74 % )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two ( 81 % ) of the patients ovulated according to basal body temperature and progesterone values , and 20 ( 74 % ) conceived during one to four treatment cycles .
	manualset3
194127	6	415828	7	NULL	NULL	0	NULL	 one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two ( 81 % ) of the patients ovulated according to basal body temperature and progesterone values , and 20 ( 74 % ) conceived during one to four treatment cycles .
	manualset3
194128	7	415828	7	NULL	NULL	0	NULL	 four treatment cycles	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two ( 81 % ) of the patients ovulated according to basal body temperature and progesterone values , and 20 ( 74 % ) conceived during one to four treatment cycles .
	manualset3
194129	1	415829	7	NULL	NULL	0	NULL	Twenty-two species	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two species of nitrogen cage molecules N ( 2n ) ( N6 ( D ( 3h ) ) , N8 ( Oh ) , N10 ( D ( 5h ) ) , N12 ( D ( 6h ) ) , N12 ( D ( 3d ) ) , N16 ( D ( 4d ) ) , N18 ( D ( 3h ) ) , N20 ( Ih ) , N24 ( D ( 3d ) ) , N24 ( D ( 4h ) ) , N24 ( D ( 6d ) ) , N30 ( D ( 3h ) ) , N30 ( D ( 5h ) ) , N32 ( D ( 4d ) ) , N36 ( D ( 3d ) ) , N40 ( D ( 4h ) ) , N42 ( D ( 3h ) ) , N48 ( D ( 4d ) ) , N48 ( D ( 3d ) ) , N54 ( D ( 3h ) ) , N56 ( D ( 4h ) ) , and N60 ( D ( 3d ) ) ) , which are divided into four sets , have been studied in detail .
	manualset3
194130	2	415829	7	NULL	NULL	0	NULL	nitrogen cage molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two species of nitrogen cage molecules N ( 2n ) ( N6 ( D ( 3h ) ) , N8 ( Oh ) , N10 ( D ( 5h ) ) , N12 ( D ( 6h ) ) , N12 ( D ( 3d ) ) , N16 ( D ( 4d ) ) , N18 ( D ( 3h ) ) , N20 ( Ih ) , N24 ( D ( 3d ) ) , N24 ( D ( 4h ) ) , N24 ( D ( 6d ) ) , N30 ( D ( 3h ) ) , N30 ( D ( 5h ) ) , N32 ( D ( 4d ) ) , N36 ( D ( 3d ) ) , N40 ( D ( 4h ) ) , N42 ( D ( 3h ) ) , N48 ( D ( 4d ) ) , N48 ( D ( 3d ) ) , N54 ( D ( 3h ) ) , N56 ( D ( 4h ) ) , and N60 ( D ( 3d ) ) ) , which are divided into four sets , have been studied in detail .
	manualset3
194131	3	415829	7	NULL	NULL	0	NULL	N ( 2n ) ( N6 ( D ( 3h ) )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two species of nitrogen cage molecules N ( 2n ) ( N6 ( D ( 3h ) ) , N8 ( Oh ) , N10 ( D ( 5h ) ) , N12 ( D ( 6h ) ) , N12 ( D ( 3d ) ) , N16 ( D ( 4d ) ) , N18 ( D ( 3h ) ) , N20 ( Ih ) , N24 ( D ( 3d ) ) , N24 ( D ( 4h ) ) , N24 ( D ( 6d ) ) , N30 ( D ( 3h ) ) , N30 ( D ( 5h ) ) , N32 ( D ( 4d ) ) , N36 ( D ( 3d ) ) , N40 ( D ( 4h ) ) , N42 ( D ( 3h ) ) , N48 ( D ( 4d ) ) , N48 ( D ( 3d ) ) , N54 ( D ( 3h ) ) , N56 ( D ( 4h ) ) , and N60 ( D ( 3d ) ) ) , which are divided into four sets , have been studied in detail .
	manualset3
194132	4	415829	7	NULL	NULL	0	NULL	N8 ( Oh ) , N10 ( D ( 5h ) )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two species of nitrogen cage molecules N ( 2n ) ( N6 ( D ( 3h ) ) , N8 ( Oh ) , N10 ( D ( 5h ) ) , N12 ( D ( 6h ) ) , N12 ( D ( 3d ) ) , N16 ( D ( 4d ) ) , N18 ( D ( 3h ) ) , N20 ( Ih ) , N24 ( D ( 3d ) ) , N24 ( D ( 4h ) ) , N24 ( D ( 6d ) ) , N30 ( D ( 3h ) ) , N30 ( D ( 5h ) ) , N32 ( D ( 4d ) ) , N36 ( D ( 3d ) ) , N40 ( D ( 4h ) ) , N42 ( D ( 3h ) ) , N48 ( D ( 4d ) ) , N48 ( D ( 3d ) ) , N54 ( D ( 3h ) ) , N56 ( D ( 4h ) ) , and N60 ( D ( 3d ) ) ) , which are divided into four sets , have been studied in detail .
	manualset3
194133	5	415829	7	NULL	NULL	0	NULL	N12 ( D ( 6h ) )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two species of nitrogen cage molecules N ( 2n ) ( N6 ( D ( 3h ) ) , N8 ( Oh ) , N10 ( D ( 5h ) ) , N12 ( D ( 6h ) ) , N12 ( D ( 3d ) ) , N16 ( D ( 4d ) ) , N18 ( D ( 3h ) ) , N20 ( Ih ) , N24 ( D ( 3d ) ) , N24 ( D ( 4h ) ) , N24 ( D ( 6d ) ) , N30 ( D ( 3h ) ) , N30 ( D ( 5h ) ) , N32 ( D ( 4d ) ) , N36 ( D ( 3d ) ) , N40 ( D ( 4h ) ) , N42 ( D ( 3h ) ) , N48 ( D ( 4d ) ) , N48 ( D ( 3d ) ) , N54 ( D ( 3h ) ) , N56 ( D ( 4h ) ) , and N60 ( D ( 3d ) ) ) , which are divided into four sets , have been studied in detail .
	manualset3
194134	6	415829	7	NULL	NULL	0	NULL	N12 ( D ( 3d ) )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two species of nitrogen cage molecules N ( 2n ) ( N6 ( D ( 3h ) ) , N8 ( Oh ) , N10 ( D ( 5h ) ) , N12 ( D ( 6h ) ) , N12 ( D ( 3d ) ) , N16 ( D ( 4d ) ) , N18 ( D ( 3h ) ) , N20 ( Ih ) , N24 ( D ( 3d ) ) , N24 ( D ( 4h ) ) , N24 ( D ( 6d ) ) , N30 ( D ( 3h ) ) , N30 ( D ( 5h ) ) , N32 ( D ( 4d ) ) , N36 ( D ( 3d ) ) , N40 ( D ( 4h ) ) , N42 ( D ( 3h ) ) , N48 ( D ( 4d ) ) , N48 ( D ( 3d ) ) , N54 ( D ( 3h ) ) , N56 ( D ( 4h ) ) , and N60 ( D ( 3d ) ) ) , which are divided into four sets , have been studied in detail .
	manualset3
194135	7	415829	7	NULL	NULL	0	NULL	N16 ( D ( 4d ) )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two species of nitrogen cage molecules N ( 2n ) ( N6 ( D ( 3h ) ) , N8 ( Oh ) , N10 ( D ( 5h ) ) , N12 ( D ( 6h ) ) , N12 ( D ( 3d ) ) , N16 ( D ( 4d ) ) , N18 ( D ( 3h ) ) , N20 ( Ih ) , N24 ( D ( 3d ) ) , N24 ( D ( 4h ) ) , N24 ( D ( 6d ) ) , N30 ( D ( 3h ) ) , N30 ( D ( 5h ) ) , N32 ( D ( 4d ) ) , N36 ( D ( 3d ) ) , N40 ( D ( 4h ) ) , N42 ( D ( 3h ) ) , N48 ( D ( 4d ) ) , N48 ( D ( 3d ) ) , N54 ( D ( 3h ) ) , N56 ( D ( 4h ) ) , and N60 ( D ( 3d ) ) ) , which are divided into four sets , have been studied in detail .
	manualset3
194137	8	415829	7	NULL	NULL	0	NULL	N18 ( D ( 3h ) )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two species of nitrogen cage molecules N ( 2n ) ( N6 ( D ( 3h ) ) , N8 ( Oh ) , N10 ( D ( 5h ) ) , N12 ( D ( 6h ) ) , N12 ( D ( 3d ) ) , N16 ( D ( 4d ) ) , N18 ( D ( 3h ) ) , N20 ( Ih ) , N24 ( D ( 3d ) ) , N24 ( D ( 4h ) ) , N24 ( D ( 6d ) ) , N30 ( D ( 3h ) ) , N30 ( D ( 5h ) ) , N32 ( D ( 4d ) ) , N36 ( D ( 3d ) ) , N40 ( D ( 4h ) ) , N42 ( D ( 3h ) ) , N48 ( D ( 4d ) ) , N48 ( D ( 3d ) ) , N54 ( D ( 3h ) ) , N56 ( D ( 4h ) ) , and N60 ( D ( 3d ) ) ) , which are divided into four sets , have been studied in detail .
	manualset3
194140	9	415829	7	NULL	NULL	0	NULL	N20 ( Ih )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two species of nitrogen cage molecules N ( 2n ) ( N6 ( D ( 3h ) ) , N8 ( Oh ) , N10 ( D ( 5h ) ) , N12 ( D ( 6h ) ) , N12 ( D ( 3d ) ) , N16 ( D ( 4d ) ) , N18 ( D ( 3h ) ) , N20 ( Ih ) , N24 ( D ( 3d ) ) , N24 ( D ( 4h ) ) , N24 ( D ( 6d ) ) , N30 ( D ( 3h ) ) , N30 ( D ( 5h ) ) , N32 ( D ( 4d ) ) , N36 ( D ( 3d ) ) , N40 ( D ( 4h ) ) , N42 ( D ( 3h ) ) , N48 ( D ( 4d ) ) , N48 ( D ( 3d ) ) , N54 ( D ( 3h ) ) , N56 ( D ( 4h ) ) , and N60 ( D ( 3d ) ) ) , which are divided into four sets , have been studied in detail .
	manualset3
194141	10	415829	7	NULL	NULL	0	NULL	N24 ( D ( 3d ) )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two species of nitrogen cage molecules N ( 2n ) ( N6 ( D ( 3h ) ) , N8 ( Oh ) , N10 ( D ( 5h ) ) , N12 ( D ( 6h ) ) , N12 ( D ( 3d ) ) , N16 ( D ( 4d ) ) , N18 ( D ( 3h ) ) , N20 ( Ih ) , N24 ( D ( 3d ) ) , N24 ( D ( 4h ) ) , N24 ( D ( 6d ) ) , N30 ( D ( 3h ) ) , N30 ( D ( 5h ) ) , N32 ( D ( 4d ) ) , N36 ( D ( 3d ) ) , N40 ( D ( 4h ) ) , N42 ( D ( 3h ) ) , N48 ( D ( 4d ) ) , N48 ( D ( 3d ) ) , N54 ( D ( 3h ) ) , N56 ( D ( 4h ) ) , and N60 ( D ( 3d ) ) ) , which are divided into four sets , have been studied in detail .
	manualset3
194142	11	415829	7	NULL	NULL	0	NULL	N24 ( D ( 4h ) )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two species of nitrogen cage molecules N ( 2n ) ( N6 ( D ( 3h ) ) , N8 ( Oh ) , N10 ( D ( 5h ) ) , N12 ( D ( 6h ) ) , N12 ( D ( 3d ) ) , N16 ( D ( 4d ) ) , N18 ( D ( 3h ) ) , N20 ( Ih ) , N24 ( D ( 3d ) ) , N24 ( D ( 4h ) ) , N24 ( D ( 6d ) ) , N30 ( D ( 3h ) ) , N30 ( D ( 5h ) ) , N32 ( D ( 4d ) ) , N36 ( D ( 3d ) ) , N40 ( D ( 4h ) ) , N42 ( D ( 3h ) ) , N48 ( D ( 4d ) ) , N48 ( D ( 3d ) ) , N54 ( D ( 3h ) ) , N56 ( D ( 4h ) ) , and N60 ( D ( 3d ) ) ) , which are divided into four sets , have been studied in detail .
	manualset3
194143	12	415829	7	NULL	NULL	0	NULL	N24 ( D ( 6d ) )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two species of nitrogen cage molecules N ( 2n ) ( N6 ( D ( 3h ) ) , N8 ( Oh ) , N10 ( D ( 5h ) ) , N12 ( D ( 6h ) ) , N12 ( D ( 3d ) ) , N16 ( D ( 4d ) ) , N18 ( D ( 3h ) ) , N20 ( Ih ) , N24 ( D ( 3d ) ) , N24 ( D ( 4h ) ) , N24 ( D ( 6d ) ) , N30 ( D ( 3h ) ) , N30 ( D ( 5h ) ) , N32 ( D ( 4d ) ) , N36 ( D ( 3d ) ) , N40 ( D ( 4h ) ) , N42 ( D ( 3h ) ) , N48 ( D ( 4d ) ) , N48 ( D ( 3d ) ) , N54 ( D ( 3h ) ) , N56 ( D ( 4h ) ) , and N60 ( D ( 3d ) ) ) , which are divided into four sets , have been studied in detail .
	manualset3
194144	13	415829	7	NULL	NULL	0	NULL	N30 ( D ( 3h ) )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two species of nitrogen cage molecules N ( 2n ) ( N6 ( D ( 3h ) ) , N8 ( Oh ) , N10 ( D ( 5h ) ) , N12 ( D ( 6h ) ) , N12 ( D ( 3d ) ) , N16 ( D ( 4d ) ) , N18 ( D ( 3h ) ) , N20 ( Ih ) , N24 ( D ( 3d ) ) , N24 ( D ( 4h ) ) , N24 ( D ( 6d ) ) , N30 ( D ( 3h ) ) , N30 ( D ( 5h ) ) , N32 ( D ( 4d ) ) , N36 ( D ( 3d ) ) , N40 ( D ( 4h ) ) , N42 ( D ( 3h ) ) , N48 ( D ( 4d ) ) , N48 ( D ( 3d ) ) , N54 ( D ( 3h ) ) , N56 ( D ( 4h ) ) , and N60 ( D ( 3d ) ) ) , which are divided into four sets , have been studied in detail .
	manualset3
194145	14	415829	7	NULL	NULL	0	NULL	N30 ( D ( 5h ) )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two species of nitrogen cage molecules N ( 2n ) ( N6 ( D ( 3h ) ) , N8 ( Oh ) , N10 ( D ( 5h ) ) , N12 ( D ( 6h ) ) , N12 ( D ( 3d ) ) , N16 ( D ( 4d ) ) , N18 ( D ( 3h ) ) , N20 ( Ih ) , N24 ( D ( 3d ) ) , N24 ( D ( 4h ) ) , N24 ( D ( 6d ) ) , N30 ( D ( 3h ) ) , N30 ( D ( 5h ) ) , N32 ( D ( 4d ) ) , N36 ( D ( 3d ) ) , N40 ( D ( 4h ) ) , N42 ( D ( 3h ) ) , N48 ( D ( 4d ) ) , N48 ( D ( 3d ) ) , N54 ( D ( 3h ) ) , N56 ( D ( 4h ) ) , and N60 ( D ( 3d ) ) ) , which are divided into four sets , have been studied in detail .
	manualset3
194146	15	415829	7	NULL	NULL	0	NULL	N32 ( D ( 4d ) )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two species of nitrogen cage molecules N ( 2n ) ( N6 ( D ( 3h ) ) , N8 ( Oh ) , N10 ( D ( 5h ) ) , N12 ( D ( 6h ) ) , N12 ( D ( 3d ) ) , N16 ( D ( 4d ) ) , N18 ( D ( 3h ) ) , N20 ( Ih ) , N24 ( D ( 3d ) ) , N24 ( D ( 4h ) ) , N24 ( D ( 6d ) ) , N30 ( D ( 3h ) ) , N30 ( D ( 5h ) ) , N32 ( D ( 4d ) ) , N36 ( D ( 3d ) ) , N40 ( D ( 4h ) ) , N42 ( D ( 3h ) ) , N48 ( D ( 4d ) ) , N48 ( D ( 3d ) ) , N54 ( D ( 3h ) ) , N56 ( D ( 4h ) ) , and N60 ( D ( 3d ) ) ) , which are divided into four sets , have been studied in detail .
	manualset3
194147	16	415829	7	NULL	NULL	0	NULL	N36 ( D ( 3d ) )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two species of nitrogen cage molecules N ( 2n ) ( N6 ( D ( 3h ) ) , N8 ( Oh ) , N10 ( D ( 5h ) ) , N12 ( D ( 6h ) ) , N12 ( D ( 3d ) ) , N16 ( D ( 4d ) ) , N18 ( D ( 3h ) ) , N20 ( Ih ) , N24 ( D ( 3d ) ) , N24 ( D ( 4h ) ) , N24 ( D ( 6d ) ) , N30 ( D ( 3h ) ) , N30 ( D ( 5h ) ) , N32 ( D ( 4d ) ) , N36 ( D ( 3d ) ) , N40 ( D ( 4h ) ) , N42 ( D ( 3h ) ) , N48 ( D ( 4d ) ) , N48 ( D ( 3d ) ) , N54 ( D ( 3h ) ) , N56 ( D ( 4h ) ) , and N60 ( D ( 3d ) ) ) , which are divided into four sets , have been studied in detail .
	manualset3
194148	17	415829	7	NULL	NULL	0	NULL	N40 ( D ( 4h ) )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two species of nitrogen cage molecules N ( 2n ) ( N6 ( D ( 3h ) ) , N8 ( Oh ) , N10 ( D ( 5h ) ) , N12 ( D ( 6h ) ) , N12 ( D ( 3d ) ) , N16 ( D ( 4d ) ) , N18 ( D ( 3h ) ) , N20 ( Ih ) , N24 ( D ( 3d ) ) , N24 ( D ( 4h ) ) , N24 ( D ( 6d ) ) , N30 ( D ( 3h ) ) , N30 ( D ( 5h ) ) , N32 ( D ( 4d ) ) , N36 ( D ( 3d ) ) , N40 ( D ( 4h ) ) , N42 ( D ( 3h ) ) , N48 ( D ( 4d ) ) , N48 ( D ( 3d ) ) , N54 ( D ( 3h ) ) , N56 ( D ( 4h ) ) , and N60 ( D ( 3d ) ) ) , which are divided into four sets , have been studied in detail .
	manualset3
194149	18	415829	7	NULL	NULL	0	NULL	N42 ( D ( 3h ) )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two species of nitrogen cage molecules N ( 2n ) ( N6 ( D ( 3h ) ) , N8 ( Oh ) , N10 ( D ( 5h ) ) , N12 ( D ( 6h ) ) , N12 ( D ( 3d ) ) , N16 ( D ( 4d ) ) , N18 ( D ( 3h ) ) , N20 ( Ih ) , N24 ( D ( 3d ) ) , N24 ( D ( 4h ) ) , N24 ( D ( 6d ) ) , N30 ( D ( 3h ) ) , N30 ( D ( 5h ) ) , N32 ( D ( 4d ) ) , N36 ( D ( 3d ) ) , N40 ( D ( 4h ) ) , N42 ( D ( 3h ) ) , N48 ( D ( 4d ) ) , N48 ( D ( 3d ) ) , N54 ( D ( 3h ) ) , N56 ( D ( 4h ) ) , and N60 ( D ( 3d ) ) ) , which are divided into four sets , have been studied in detail .
	manualset3
194150	19	415829	7	NULL	NULL	0	NULL	N48 ( D ( 4d ) ) 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two species of nitrogen cage molecules N ( 2n ) ( N6 ( D ( 3h ) ) , N8 ( Oh ) , N10 ( D ( 5h ) ) , N12 ( D ( 6h ) ) , N12 ( D ( 3d ) ) , N16 ( D ( 4d ) ) , N18 ( D ( 3h ) ) , N20 ( Ih ) , N24 ( D ( 3d ) ) , N24 ( D ( 4h ) ) , N24 ( D ( 6d ) ) , N30 ( D ( 3h ) ) , N30 ( D ( 5h ) ) , N32 ( D ( 4d ) ) , N36 ( D ( 3d ) ) , N40 ( D ( 4h ) ) , N42 ( D ( 3h ) ) , N48 ( D ( 4d ) ) , N48 ( D ( 3d ) ) , N54 ( D ( 3h ) ) , N56 ( D ( 4h ) ) , and N60 ( D ( 3d ) ) ) , which are divided into four sets , have been studied in detail .
	manualset3
194151	20	415829	7	NULL	NULL	0	NULL	 N48 ( D ( 3d ) )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two species of nitrogen cage molecules N ( 2n ) ( N6 ( D ( 3h ) ) , N8 ( Oh ) , N10 ( D ( 5h ) ) , N12 ( D ( 6h ) ) , N12 ( D ( 3d ) ) , N16 ( D ( 4d ) ) , N18 ( D ( 3h ) ) , N20 ( Ih ) , N24 ( D ( 3d ) ) , N24 ( D ( 4h ) ) , N24 ( D ( 6d ) ) , N30 ( D ( 3h ) ) , N30 ( D ( 5h ) ) , N32 ( D ( 4d ) ) , N36 ( D ( 3d ) ) , N40 ( D ( 4h ) ) , N42 ( D ( 3h ) ) , N48 ( D ( 4d ) ) , N48 ( D ( 3d ) ) , N54 ( D ( 3h ) ) , N56 ( D ( 4h ) ) , and N60 ( D ( 3d ) ) ) , which are divided into four sets , have been studied in detail .
	manualset3
194152	21	415829	7	NULL	NULL	0	NULL	N54 ( D ( 3h ) )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two species of nitrogen cage molecules N ( 2n ) ( N6 ( D ( 3h ) ) , N8 ( Oh ) , N10 ( D ( 5h ) ) , N12 ( D ( 6h ) ) , N12 ( D ( 3d ) ) , N16 ( D ( 4d ) ) , N18 ( D ( 3h ) ) , N20 ( Ih ) , N24 ( D ( 3d ) ) , N24 ( D ( 4h ) ) , N24 ( D ( 6d ) ) , N30 ( D ( 3h ) ) , N30 ( D ( 5h ) ) , N32 ( D ( 4d ) ) , N36 ( D ( 3d ) ) , N40 ( D ( 4h ) ) , N42 ( D ( 3h ) ) , N48 ( D ( 4d ) ) , N48 ( D ( 3d ) ) , N54 ( D ( 3h ) ) , N56 ( D ( 4h ) ) , and N60 ( D ( 3d ) ) ) , which are divided into four sets , have been studied in detail .
	manualset3
194153	22	415829	7	NULL	NULL	0	NULL	N56 ( D ( 4h ) )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two species of nitrogen cage molecules N ( 2n ) ( N6 ( D ( 3h ) ) , N8 ( Oh ) , N10 ( D ( 5h ) ) , N12 ( D ( 6h ) ) , N12 ( D ( 3d ) ) , N16 ( D ( 4d ) ) , N18 ( D ( 3h ) ) , N20 ( Ih ) , N24 ( D ( 3d ) ) , N24 ( D ( 4h ) ) , N24 ( D ( 6d ) ) , N30 ( D ( 3h ) ) , N30 ( D ( 5h ) ) , N32 ( D ( 4d ) ) , N36 ( D ( 3d ) ) , N40 ( D ( 4h ) ) , N42 ( D ( 3h ) ) , N48 ( D ( 4d ) ) , N48 ( D ( 3d ) ) , N54 ( D ( 3h ) ) , N56 ( D ( 4h ) ) , and N60 ( D ( 3d ) ) ) , which are divided into four sets , have been studied in detail .
	manualset3
194154	23	415829	7	NULL	NULL	0	NULL	N60 ( D ( 3d ) ) )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two species of nitrogen cage molecules N ( 2n ) ( N6 ( D ( 3h ) ) , N8 ( Oh ) , N10 ( D ( 5h ) ) , N12 ( D ( 6h ) ) , N12 ( D ( 3d ) ) , N16 ( D ( 4d ) ) , N18 ( D ( 3h ) ) , N20 ( Ih ) , N24 ( D ( 3d ) ) , N24 ( D ( 4h ) ) , N24 ( D ( 6d ) ) , N30 ( D ( 3h ) ) , N30 ( D ( 5h ) ) , N32 ( D ( 4d ) ) , N36 ( D ( 3d ) ) , N40 ( D ( 4h ) ) , N42 ( D ( 3h ) ) , N48 ( D ( 4d ) ) , N48 ( D ( 3d ) ) , N54 ( D ( 3h ) ) , N56 ( D ( 4h ) ) , and N60 ( D ( 3d ) ) ) , which are divided into four sets , have been studied in detail .
	manualset3
194155	24	415829	7	NULL	NULL	0	NULL	four sets	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-two species of nitrogen cage molecules N ( 2n ) ( N6 ( D ( 3h ) ) , N8 ( Oh ) , N10 ( D ( 5h ) ) , N12 ( D ( 6h ) ) , N12 ( D ( 3d ) ) , N16 ( D ( 4d ) ) , N18 ( D ( 3h ) ) , N20 ( Ih ) , N24 ( D ( 3d ) ) , N24 ( D ( 4h ) ) , N24 ( D ( 6d ) ) , N30 ( D ( 3h ) ) , N30 ( D ( 5h ) ) , N32 ( D ( 4d ) ) , N36 ( D ( 3d ) ) , N40 ( D ( 4h ) ) , N42 ( D ( 3h ) ) , N48 ( D ( 4d ) ) , N48 ( D ( 3d ) ) , N54 ( D ( 3h ) ) , N56 ( D ( 4h ) ) , and N60 ( D ( 3d ) ) ) , which are divided into four sets , have been studied in detail .
	manualset3
194156	1	415830	7	NULL	NULL	0	NULL	oxidopamine treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After oxidopamine treatment , rats had a higher survival rate and greater pancreatic blood flow than untreated controls .
	manualset3
194157	2	415830	7	NULL	NULL	0	NULL	 rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	After oxidopamine treatment , rats had a higher survival rate and greater pancreatic blood flow than untreated controls .
	manualset3
194158	3	415830	7	NULL	NULL	0	NULL	higher survival rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After oxidopamine treatment , rats had a higher survival rate and greater pancreatic blood flow than untreated controls .
	manualset3
194159	4	415830	7	NULL	NULL	0	NULL	pancreatic blood flow	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After oxidopamine treatment , rats had a higher survival rate and greater pancreatic blood flow than untreated controls .
	manualset3
194160	5	415830	7	NULL	NULL	0	NULL	untreated controls	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	After oxidopamine treatment , rats had a higher survival rate and greater pancreatic blood flow than untreated controls .
	manualset3
194270	1	415831	7	NULL	NULL	0	NULL	Twenty basis vectors	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty basis vectors are employed for these calculations , and the corresponding effective potential energy surfaces are identified in the asymptotic limit by the H2 rotor quantum numbers j = 0 , 2 , 4 , 6 and B electronic states 2Pja , ja = 1/2 , 3/2 .
	manualset3
194271	2	415831	7	NULL	NULL	0	NULL	calculations	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty basis vectors are employed for these calculations , and the corresponding effective potential energy surfaces are identified in the asymptotic limit by the H2 rotor quantum numbers j = 0 , 2 , 4 , 6 and B electronic states 2Pja , ja = 1/2 , 3/2 .
	manualset3
194272	3	415831	7	NULL	NULL	0	NULL	potential energy surfaces	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty basis vectors are employed for these calculations , and the corresponding effective potential energy surfaces are identified in the asymptotic limit by the H2 rotor quantum numbers j = 0 , 2 , 4 , 6 and B electronic states 2Pja , ja = 1/2 , 3/2 .
	manualset3
194273	4	415831	7	NULL	NULL	0	NULL	asymptotic limit	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty basis vectors are employed for these calculations , and the corresponding effective potential energy surfaces are identified in the asymptotic limit by the H2 rotor quantum numbers j = 0 , 2 , 4 , 6 and B electronic states 2Pja , ja = 1/2 , 3/2 .
	manualset3
194274	5	415831	7	NULL	NULL	NULL	NULL	H2 rotor quantum numbers	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Twenty basis vectors are employed for these calculations , and the corresponding effective potential energy surfaces are identified in the asymptotic limit by the H2 rotor quantum numbers j = 0 , 2 , 4 , 6 and B electronic states 2Pja , ja = 1/2 , 3/2 .
	manualset3
194275	6	415831	7	NULL	NULL	0	NULL	j = 0 , 2 , 4 , 6	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty basis vectors are employed for these calculations , and the corresponding effective potential energy surfaces are identified in the asymptotic limit by the H2 rotor quantum numbers j = 0 , 2 , 4 , 6 and B electronic states 2Pja , ja = 1/2 , 3/2 .
	manualset3
194276	7	415831	7	NULL	NULL	0	NULL	B electronic states 2Pja	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty basis vectors are employed for these calculations , and the corresponding effective potential energy surfaces are identified in the asymptotic limit by the H2 rotor quantum numbers j = 0 , 2 , 4 , 6 and B electronic states 2Pja , ja = 1/2 , 3/2 .
	manualset3
194277	8	415831	7	NULL	NULL	0	NULL	ja = 1/2 , 3/2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty basis vectors are employed for these calculations , and the corresponding effective potential energy surfaces are identified in the asymptotic limit by the H2 rotor quantum numbers j = 0 , 2 , 4 , 6 and B electronic states 2Pja , ja = 1/2 , 3/2 .
	manualset3
194278	1	415832	7	NULL	NULL	0	NULL	Twenty children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty children with type 1 diabetes ( 12 boys/8 girls , age 12-15 yr ) performed 29 exercise studies ( 30-min intermittent cycling at approximately 80 % peak O2 uptake ) .
	manualset3
194279	2	415832	7	NULL	NULL	0	NULL	type 1 diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty children with type 1 diabetes ( 12 boys/8 girls , age 12-15 yr ) performed 29 exercise studies ( 30-min intermittent cycling at approximately 80 % peak O2 uptake ) .
	manualset3
194280	3	415832	7	NULL	NULL	0	NULL	12 boys/8 girls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty children with type 1 diabetes ( 12 boys/8 girls , age 12-15 yr ) performed 29 exercise studies ( 30-min intermittent cycling at approximately 80 % peak O2 uptake ) .
	manualset3
194281	4	415832	7	NULL	NULL	0	NULL	age 12-15 yr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty children with type 1 diabetes ( 12 boys/8 girls , age 12-15 yr ) performed 29 exercise studies ( 30-min intermittent cycling at approximately 80 % peak O2 uptake ) .
	manualset3
194282	5	415832	7	NULL	NULL	0	NULL	29 exercise studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty children with type 1 diabetes ( 12 boys/8 girls , age 12-15 yr ) performed 29 exercise studies ( 30-min intermittent cycling at approximately 80 % peak O2 uptake ) .
	manualset3
194283	6	415832	7	NULL	NULL	0	NULL	30-min intermittent cycling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty children with type 1 diabetes ( 12 boys/8 girls , age 12-15 yr ) performed 29 exercise studies ( 30-min intermittent cycling at approximately 80 % peak O2 uptake ) .
	manualset3
194284	7	415832	7	NULL	NULL	0	NULL	80 % peak	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty children with type 1 diabetes ( 12 boys/8 girls , age 12-15 yr ) performed 29 exercise studies ( 30-min intermittent cycling at approximately 80 % peak O2 uptake ) .
	manualset3
194285	8	415832	7	NULL	NULL	0	NULL	O2 uptake 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty children with type 1 diabetes ( 12 boys/8 girls , age 12-15 yr ) performed 29 exercise studies ( 30-min intermittent cycling at approximately 80 % peak O2 uptake ) .
	manualset3
194286	1	415833	7	NULL	NULL	0	NULL	Twenty consecutive patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty consecutive patients with untreated brain arteriovenous malformations were recruited ( 10 with and 10 without epileptic seizures ) along with 12 age-matched healthy controls .
	manualset3
194287	2	415833	7	NULL	NULL	0	NULL	untreated brain arteriovenous malformations	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty consecutive patients with untreated brain arteriovenous malformations were recruited ( 10 with and 10 without epileptic seizures ) along with 12 age-matched healthy controls .
	manualset3
194288	3	415833	7	NULL	NULL	0	NULL	10 with epileptic seizures	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty consecutive patients with untreated brain arteriovenous malformations were recruited ( 10 with and 10 without epileptic seizures ) along with 12 age-matched healthy controls .
	manualset3
194289	4	415833	7	NULL	NULL	0	NULL	10 without epileptic seizures	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty consecutive patients with untreated brain arteriovenous malformations were recruited ( 10 with and 10 without epileptic seizures ) along with 12 age-matched healthy controls .
	manualset3
194290	5	415833	7	NULL	NULL	0	NULL	12 age-matched healthy controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty consecutive patients with untreated brain arteriovenous malformations were recruited ( 10 with and 10 without epileptic seizures ) along with 12 age-matched healthy controls .
	manualset3
194291	1	415834	7	NULL	NULL	0	NULL	Twenty days post abortion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty days post abortion the llama was rebred .
	manualset3
194292	2	415834	7	NULL	NULL	0	NULL	 llama	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty days post abortion the llama was rebred .
	manualset3
194293	1	415835	7	NULL	NULL	0	NULL	Twenty hours 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty hours after the last of 7 daily injections of ( + ) - amphetamine ( 5 mg kg-1 i.p. ) the concentration of alpha-methyl-p-tyramine in striatal tissue increased twofold compared to the concentration 20 h after a single injection .
	manualset3
194294	2	415835	7	NULL	NULL	NULL	NULL	last	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Twenty hours after the last of 7 daily injections of ( + ) - amphetamine ( 5 mg kg-1 i.p. ) the concentration of alpha-methyl-p-tyramine in striatal tissue increased twofold compared to the concentration 20 h after a single injection .
	manualset3
194295	3	415835	7	NULL	NULL	0	NULL	7 daily injections	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty hours after the last of 7 daily injections of ( + ) - amphetamine ( 5 mg kg-1 i.p. ) the concentration of alpha-methyl-p-tyramine in striatal tissue increased twofold compared to the concentration 20 h after a single injection .
	manualset3
194296	4	415835	7	NULL	NULL	0	NULL	( + ) - amphetamine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty hours after the last of 7 daily injections of ( + ) - amphetamine ( 5 mg kg-1 i.p. ) the concentration of alpha-methyl-p-tyramine in striatal tissue increased twofold compared to the concentration 20 h after a single injection .
	manualset3
194297	5	415835	7	NULL	NULL	0	NULL	5 mg kg-1 i.p.	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty hours after the last of 7 daily injections of ( + ) - amphetamine ( 5 mg kg-1 i.p. ) the concentration of alpha-methyl-p-tyramine in striatal tissue increased twofold compared to the concentration 20 h after a single injection .
	manualset3
194298	6	415835	7	NULL	NULL	0	NULL	concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty hours after the last of 7 daily injections of ( + ) - amphetamine ( 5 mg kg-1 i.p. ) the concentration of alpha-methyl-p-tyramine in striatal tissue increased twofold compared to the concentration 20 h after a single injection .
	manualset3
194299	7	415835	7	NULL	NULL	0	NULL	alpha-methyl-p-tyramine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty hours after the last of 7 daily injections of ( + ) - amphetamine ( 5 mg kg-1 i.p. ) the concentration of alpha-methyl-p-tyramine in striatal tissue increased twofold compared to the concentration 20 h after a single injection .
	manualset3
194300	8	415835	7	NULL	NULL	0	NULL	 striatal tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty hours after the last of 7 daily injections of ( + ) - amphetamine ( 5 mg kg-1 i.p. ) the concentration of alpha-methyl-p-tyramine in striatal tissue increased twofold compared to the concentration 20 h after a single injection .
	manualset3
194301	9	415835	7	NULL	NULL	0	NULL	twofold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty hours after the last of 7 daily injections of ( + ) - amphetamine ( 5 mg kg-1 i.p. ) the concentration of alpha-methyl-p-tyramine in striatal tissue increased twofold compared to the concentration 20 h after a single injection .
	manualset3
194302	10	415835	7	NULL	NULL	0	NULL	concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty hours after the last of 7 daily injections of ( + ) - amphetamine ( 5 mg kg-1 i.p. ) the concentration of alpha-methyl-p-tyramine in striatal tissue increased twofold compared to the concentration 20 h after a single injection .
	manualset3
194303	11	415835	7	NULL	NULL	0	NULL	20 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty hours after the last of 7 daily injections of ( + ) - amphetamine ( 5 mg kg-1 i.p. ) the concentration of alpha-methyl-p-tyramine in striatal tissue increased twofold compared to the concentration 20 h after a single injection .
	manualset3
194304	12	415835	7	NULL	NULL	0	NULL	single injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty hours after the last of 7 daily injections of ( + ) - amphetamine ( 5 mg kg-1 i.p. ) the concentration of alpha-methyl-p-tyramine in striatal tissue increased twofold compared to the concentration 20 h after a single injection .
	manualset3
194305	1	415836	7	NULL	NULL	0	NULL	Twenty inpatients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty inpatients with schizophrenia were administered fixed doses of neuroleptics throughout the study .
	manualset3
194306	2	415836	7	NULL	NULL	0	NULL	schizophrenia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty inpatients with schizophrenia were administered fixed doses of neuroleptics throughout the study .
	manualset3
194307	3	415836	7	NULL	NULL	0	NULL	fixed doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty inpatients with schizophrenia were administered fixed doses of neuroleptics throughout the study .
	manualset3
194308	4	415836	7	NULL	NULL	0	NULL	neuroleptics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty inpatients with schizophrenia were administered fixed doses of neuroleptics throughout the study .
	manualset3
194309	5	415836	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty inpatients with schizophrenia were administered fixed doses of neuroleptics throughout the study .
	manualset3
194310	1	415837	7	NULL	NULL	0	NULL	endoscopic mechanical lithotripsy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After performing endoscopic mechanical lithotripsy in patients suffering from common bile duct stones , we could improve our success rate ( stone free system ) from 89 % up to 97.4 % .
	manualset3
194311	2	415837	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	After performing endoscopic mechanical lithotripsy in patients suffering from common bile duct stones , we could improve our success rate ( stone free system ) from 89 % up to 97.4 % .
	manualset3
194312	3	415837	7	NULL	NULL	0	NULL	common bile duct stones	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After performing endoscopic mechanical lithotripsy in patients suffering from common bile duct stones , we could improve our success rate ( stone free system ) from 89 % up to 97.4 % .
	manualset3
194313	4	415837	7	NULL	NULL	0	NULL	success rate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After performing endoscopic mechanical lithotripsy in patients suffering from common bile duct stones , we could improve our success rate ( stone free system ) from 89 % up to 97.4 % .
	manualset3
194314	5	415837	7	NULL	NULL	0	NULL	stone free system	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After performing endoscopic mechanical lithotripsy in patients suffering from common bile duct stones , we could improve our success rate ( stone free system ) from 89 % up to 97.4 % .
	manualset3
194315	6	415837	7	NULL	NULL	0	NULL	89 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After performing endoscopic mechanical lithotripsy in patients suffering from common bile duct stones , we could improve our success rate ( stone free system ) from 89 % up to 97.4 % .
	manualset3
194316	7	415837	7	NULL	NULL	0	NULL	97.4 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After performing endoscopic mechanical lithotripsy in patients suffering from common bile duct stones , we could improve our success rate ( stone free system ) from 89 % up to 97.4 % .
	manualset3
194317	1	415838	7	NULL	NULL	0	NULL	Twenty participants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty participants ( 14 men ) were presented a passive oddball auditory task in which they were exposed to uniform auditory stimulation of tones with occasional deviations in tone frequency , a procedure that elicits the mismatch negativity ( MMN ) and its magnetic counterpart ( MMNm ) .
	manualset3
194318	2	415838	7	NULL	NULL	0	NULL	14 men 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty participants ( 14 men ) were presented a passive oddball auditory task in which they were exposed to uniform auditory stimulation of tones with occasional deviations in tone frequency , a procedure that elicits the mismatch negativity ( MMN ) and its magnetic counterpart ( MMNm ) .
	manualset3
194319	3	415838	7	NULL	NULL	0	NULL	passive oddball auditory task	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty participants ( 14 men ) were presented a passive oddball auditory task in which they were exposed to uniform auditory stimulation of tones with occasional deviations in tone frequency , a procedure that elicits the mismatch negativity ( MMN ) and its magnetic counterpart ( MMNm ) .
	manualset3
194320	4	415838	7	NULL	NULL	NULL	NULL	uniform auditory stimulation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Twenty participants ( 14 men ) were presented a passive oddball auditory task in which they were exposed to uniform auditory stimulation of tones with occasional deviations in tone frequency , a procedure that elicits the mismatch negativity ( MMN ) and its magnetic counterpart ( MMNm ) .
	manualset3
194321	5	415838	7	NULL	NULL	0	NULL	occasional deviations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty participants ( 14 men ) were presented a passive oddball auditory task in which they were exposed to uniform auditory stimulation of tones with occasional deviations in tone frequency , a procedure that elicits the mismatch negativity ( MMN ) and its magnetic counterpart ( MMNm ) .
	manualset3
194322	6	415838	7	NULL	NULL	0	NULL	tone frequency 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty participants ( 14 men ) were presented a passive oddball auditory task in which they were exposed to uniform auditory stimulation of tones with occasional deviations in tone frequency , a procedure that elicits the mismatch negativity ( MMN ) and its magnetic counterpart ( MMNm ) .
	manualset3
194323	7	415838	7	NULL	NULL	0	NULL	procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty participants ( 14 men ) were presented a passive oddball auditory task in which they were exposed to uniform auditory stimulation of tones with occasional deviations in tone frequency , a procedure that elicits the mismatch negativity ( MMN ) and its magnetic counterpart ( MMNm ) .
	manualset3
194325	8	415838	7	NULL	NULL	0	NULL	mismatch negativity ( MMN ) 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty participants ( 14 men ) were presented a passive oddball auditory task in which they were exposed to uniform auditory stimulation of tones with occasional deviations in tone frequency , a procedure that elicits the mismatch negativity ( MMN ) and its magnetic counterpart ( MMNm ) .
	manualset3
194326	9	415838	7	NULL	NULL	0	NULL	magnetic counterpart ( MMNm )	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty participants ( 14 men ) were presented a passive oddball auditory task in which they were exposed to uniform auditory stimulation of tones with occasional deviations in tone frequency , a procedure that elicits the mismatch negativity ( MMN ) and its magnetic counterpart ( MMNm ) .
	manualset3
194327	10	415838	7	NULL	NULL	0	NULL	tones	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty participants ( 14 men ) were presented a passive oddball auditory task in which they were exposed to uniform auditory stimulation of tones with occasional deviations in tone frequency , a procedure that elicits the mismatch negativity ( MMN ) and its magnetic counterpart ( MMNm ) .
	manualset3
194330	1	415839	7	NULL	NULL	NULL	NULL	Twenty stone cast/wax base sets	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Twenty stone cast/wax base sets were confected for routine flasking procedure .
	manualset3
194331	2	415839	7	NULL	NULL	0	NULL	 routine flasking procedure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty stone cast/wax base sets were confected for routine flasking procedure .
	manualset3
194338	1	415840	7	NULL	NULL	0	NULL	Twin reversed arterial perfusion ( TRAP ) sequence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twin reversed arterial perfusion ( TRAP ) sequence in association with VACTERL association : a case report .
	manualset3
194340	2	415840	7	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Twin reversed arterial perfusion ( TRAP ) sequence in association with VACTERL association : a case report .
	manualset3
194342	3	415840	7	NULL	NULL	0	NULL	VACTERL association	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twin reversed arterial perfusion ( TRAP ) sequence in association with VACTERL association : a case report .
	manualset3
194343	4	415840	7	NULL	NULL	0	NULL	case report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Twin reversed arterial perfusion ( TRAP ) sequence in association with VACTERL association : a case report .
	manualset3
194362	1	415841	7	NULL	NULL	0	NULL	Two-color resonant four-wave mixing spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-color resonant four-wave mixing spectroscopy of highly predissociated levels in the A 2A1 state of CH3S .
	manualset3
194363	2	415841	7	NULL	NULL	0	NULL	highly predissociated levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-color resonant four-wave mixing spectroscopy of highly predissociated levels in the A 2A1 state of CH3S .
	manualset3
194364	3	415841	7	NULL	NULL	0	NULL	A 2A1 state	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-color resonant four-wave mixing spectroscopy of highly predissociated levels in the A 2A1 state of CH3S .
	manualset3
194365	4	415841	7	NULL	NULL	0	NULL	 CH3S	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-color resonant four-wave mixing spectroscopy of highly predissociated levels in the A 2A1 state of CH3S .
	manualset3
194437	1	415842	7	NULL	NULL	0	NULL	 propagation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After propagation and cloning in cell culture , the four viruses were used to produce convalescent and hyperimmune antisera in gnotobiotic animals .
	manualset3
194438	2	415842	7	NULL	NULL	0	NULL	cloning	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After propagation and cloning in cell culture , the four viruses were used to produce convalescent and hyperimmune antisera in gnotobiotic animals .
	manualset3
194439	3	415842	7	NULL	NULL	0	NULL	cell culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	After propagation and cloning in cell culture , the four viruses were used to produce convalescent and hyperimmune antisera in gnotobiotic animals .
	manualset3
194440	4	415842	7	NULL	NULL	0	NULL	four viruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	After propagation and cloning in cell culture , the four viruses were used to produce convalescent and hyperimmune antisera in gnotobiotic animals .
	manualset3
194441	5	415842	7	NULL	NULL	0	NULL	convalescent antisera	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After propagation and cloning in cell culture , the four viruses were used to produce convalescent and hyperimmune antisera in gnotobiotic animals .
	manualset3
194442	6	415842	7	NULL	NULL	0	NULL	hyperimmune antisera 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After propagation and cloning in cell culture , the four viruses were used to produce convalescent and hyperimmune antisera in gnotobiotic animals .
	manualset3
194443	7	415842	7	NULL	NULL	0	NULL	gnotobiotic animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	After propagation and cloning in cell culture , the four viruses were used to produce convalescent and hyperimmune antisera in gnotobiotic animals .
	manualset3
194444	1	415843	7	NULL	NULL	0	NULL	Two-electrode recordings	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-electrode recordings revealed tight electrical coupling ( 83 % ) between neighboring cells in the circumferential direction of the artery .
	manualset3
194445	2	415843	7	NULL	NULL	0	NULL	tight electrical coupling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-electrode recordings revealed tight electrical coupling ( 83 % ) between neighboring cells in the circumferential direction of the artery .
	manualset3
194446	3	415843	7	NULL	NULL	NULL	NULL	83 %	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two-electrode recordings revealed tight electrical coupling ( 83 % ) between neighboring cells in the circumferential direction of the artery .
	manualset3
194447	4	415843	7	NULL	NULL	0	NULL	neighboring cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-electrode recordings revealed tight electrical coupling ( 83 % ) between neighboring cells in the circumferential direction of the artery .
	manualset3
194448	5	415843	7	NULL	NULL	0	NULL	circumferential direction	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-electrode recordings revealed tight electrical coupling ( 83 % ) between neighboring cells in the circumferential direction of the artery .
	manualset3
194449	6	415843	7	NULL	NULL	0	NULL	artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-electrode recordings revealed tight electrical coupling ( 83 % ) between neighboring cells in the circumferential direction of the artery .
	manualset3
194450	1	415844	7	NULL	NULL	0	NULL	Two-hundred and seven patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-hundred and seven patients without evidence of disease following lymph node dissection ( LND ) were stratified into three groups : Group A , lymph node relapse within the site of prior LND ; Group B , lymph node relapse in a different , but regional , lymph node group ; Group C , no lymph node relapse .
	manualset3
194451	2	415844	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-hundred and seven patients without evidence of disease following lymph node dissection ( LND ) were stratified into three groups : Group A , lymph node relapse within the site of prior LND ; Group B , lymph node relapse in a different , but regional , lymph node group ; Group C , no lymph node relapse .
	manualset3
194452	3	415844	7	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-hundred and seven patients without evidence of disease following lymph node dissection ( LND ) were stratified into three groups : Group A , lymph node relapse within the site of prior LND ; Group B , lymph node relapse in a different , but regional , lymph node group ; Group C , no lymph node relapse .
	manualset3
194453	4	415844	7	NULL	NULL	0	NULL	lymph node dissection ( LND )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-hundred and seven patients without evidence of disease following lymph node dissection ( LND ) were stratified into three groups : Group A , lymph node relapse within the site of prior LND ; Group B , lymph node relapse in a different , but regional , lymph node group ; Group C , no lymph node relapse .
	manualset3
194454	5	415844	7	NULL	NULL	0	NULL	three groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-hundred and seven patients without evidence of disease following lymph node dissection ( LND ) were stratified into three groups : Group A , lymph node relapse within the site of prior LND ; Group B , lymph node relapse in a different , but regional , lymph node group ; Group C , no lymph node relapse .
	manualset3
194455	6	415844	7	NULL	NULL	0	NULL	Group A	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-hundred and seven patients without evidence of disease following lymph node dissection ( LND ) were stratified into three groups : Group A , lymph node relapse within the site of prior LND ; Group B , lymph node relapse in a different , but regional , lymph node group ; Group C , no lymph node relapse .
	manualset3
194456	7	415844	7	NULL	NULL	NULL	NULL	lymph node relapse	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two-hundred and seven patients without evidence of disease following lymph node dissection ( LND ) were stratified into three groups : Group A , lymph node relapse within the site of prior LND ; Group B , lymph node relapse in a different , but regional , lymph node group ; Group C , no lymph node relapse .
	manualset3
194457	8	415844	7	NULL	NULL	NULL	NULL	 the site of prior LND	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two-hundred and seven patients without evidence of disease following lymph node dissection ( LND ) were stratified into three groups : Group A , lymph node relapse within the site of prior LND ; Group B , lymph node relapse in a different , but regional , lymph node group ; Group C , no lymph node relapse .
	manualset3
194459	10	415844	7	NULL	NULL	0	NULL	Group B	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-hundred and seven patients without evidence of disease following lymph node dissection ( LND ) were stratified into three groups : Group A , lymph node relapse within the site of prior LND ; Group B , lymph node relapse in a different , but regional , lymph node group ; Group C , no lymph node relapse .
	manualset3
194460	11	415844	7	NULL	NULL	0	NULL	lymph node relapse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-hundred and seven patients without evidence of disease following lymph node dissection ( LND ) were stratified into three groups : Group A , lymph node relapse within the site of prior LND ; Group B , lymph node relapse in a different , but regional , lymph node group ; Group C , no lymph node relapse .
	manualset3
194461	12	415844	7	NULL	NULL	0	NULL	regional lymph node group	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-hundred and seven patients without evidence of disease following lymph node dissection ( LND ) were stratified into three groups : Group A , lymph node relapse within the site of prior LND ; Group B , lymph node relapse in a different , but regional , lymph node group ; Group C , no lymph node relapse .
	manualset3
194462	13	415844	7	NULL	NULL	0	NULL	 Group C	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-hundred and seven patients without evidence of disease following lymph node dissection ( LND ) were stratified into three groups : Group A , lymph node relapse within the site of prior LND ; Group B , lymph node relapse in a different , but regional , lymph node group ; Group C , no lymph node relapse .
	manualset3
194463	14	415844	7	NULL	NULL	0	NULL	no lymph node relapse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-hundred and seven patients without evidence of disease following lymph node dissection ( LND ) were stratified into three groups : Group A , lymph node relapse within the site of prior LND ; Group B , lymph node relapse in a different , but regional , lymph node group ; Group C , no lymph node relapse .
	manualset3
194481	1	415845	7	NULL	NULL	0	NULL	Two-minute trains	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-minute trains of electrical pulses ( alternate polarity , 2-ms duration ; 100 mA intensity ; 10 V drop between electrodes ; frequency 5 , 10 and 20 Hz ) applied to cultures kept at 27 degrees C , elicited a D - ( 3H ) aspartate outflow which was frequency related , ( Ca2 + ) 0 dependent , tetrodotoxin sensitive .
	manualset3
194483	2	415845	7	NULL	NULL	0	NULL	electrical pulses 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-minute trains of electrical pulses ( alternate polarity , 2-ms duration ; 100 mA intensity ; 10 V drop between electrodes ; frequency 5 , 10 and 20 Hz ) applied to cultures kept at 27 degrees C , elicited a D - ( 3H ) aspartate outflow which was frequency related , ( Ca2 + ) 0 dependent , tetrodotoxin sensitive .
	manualset3
194485	3	415845	7	NULL	NULL	NULL	NULL	alternate polarity	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two-minute trains of electrical pulses ( alternate polarity , 2-ms duration ; 100 mA intensity ; 10 V drop between electrodes ; frequency 5 , 10 and 20 Hz ) applied to cultures kept at 27 degrees C , elicited a D - ( 3H ) aspartate outflow which was frequency related , ( Ca2 + ) 0 dependent , tetrodotoxin sensitive .
	manualset3
194488	4	415845	7	NULL	NULL	0	NULL	2-ms duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-minute trains of electrical pulses ( alternate polarity , 2-ms duration ; 100 mA intensity ; 10 V drop between electrodes ; frequency 5 , 10 and 20 Hz ) applied to cultures kept at 27 degrees C , elicited a D - ( 3H ) aspartate outflow which was frequency related , ( Ca2 + ) 0 dependent , tetrodotoxin sensitive .
	manualset3
194489	5	415845	7	NULL	NULL	0	NULL	100 mA intensity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-minute trains of electrical pulses ( alternate polarity , 2-ms duration ; 100 mA intensity ; 10 V drop between electrodes ; frequency 5 , 10 and 20 Hz ) applied to cultures kept at 27 degrees C , elicited a D - ( 3H ) aspartate outflow which was frequency related , ( Ca2 + ) 0 dependent , tetrodotoxin sensitive .
	manualset3
194499	6	415845	7	NULL	NULL	0	NULL	10 V drop 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-minute trains of electrical pulses ( alternate polarity , 2-ms duration ; 100 mA intensity ; 10 V drop between electrodes ; frequency 5 , 10 and 20 Hz ) applied to cultures kept at 27 degrees C , elicited a D - ( 3H ) aspartate outflow which was frequency related , ( Ca2 + ) 0 dependent , tetrodotoxin sensitive .
	manualset3
194500	7	415845	7	NULL	NULL	0	NULL	electrodes	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-minute trains of electrical pulses ( alternate polarity , 2-ms duration ; 100 mA intensity ; 10 V drop between electrodes ; frequency 5 , 10 and 20 Hz ) applied to cultures kept at 27 degrees C , elicited a D - ( 3H ) aspartate outflow which was frequency related , ( Ca2 + ) 0 dependent , tetrodotoxin sensitive .
	manualset3
194502	8	415845	7	NULL	NULL	0	NULL	frequency 5 Hz	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-minute trains of electrical pulses ( alternate polarity , 2-ms duration ; 100 mA intensity ; 10 V drop between electrodes ; frequency 5 , 10 and 20 Hz ) applied to cultures kept at 27 degrees C , elicited a D - ( 3H ) aspartate outflow which was frequency related , ( Ca2 + ) 0 dependent , tetrodotoxin sensitive .
	manualset3
194506	9	415845	7	NULL	NULL	NULL	NULL	frequency 10 Hz	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two-minute trains of electrical pulses ( alternate polarity , 2-ms duration ; 100 mA intensity ; 10 V drop between electrodes ; frequency 5 , 10 and 20 Hz ) applied to cultures kept at 27 degrees C , elicited a D - ( 3H ) aspartate outflow which was frequency related , ( Ca2 + ) 0 dependent , tetrodotoxin sensitive .
	manualset3
194511	10	415845	7	NULL	NULL	0	NULL	frequency 20 Hz	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-minute trains of electrical pulses ( alternate polarity , 2-ms duration ; 100 mA intensity ; 10 V drop between electrodes ; frequency 5 , 10 and 20 Hz ) applied to cultures kept at 27 degrees C , elicited a D - ( 3H ) aspartate outflow which was frequency related , ( Ca2 + ) 0 dependent , tetrodotoxin sensitive .
	manualset3
194518	11	415845	7	NULL	NULL	0	NULL	cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-minute trains of electrical pulses ( alternate polarity , 2-ms duration ; 100 mA intensity ; 10 V drop between electrodes ; frequency 5 , 10 and 20 Hz ) applied to cultures kept at 27 degrees C , elicited a D - ( 3H ) aspartate outflow which was frequency related , ( Ca2 + ) 0 dependent , tetrodotoxin sensitive .
	manualset3
194519	12	415845	7	NULL	NULL	0	NULL	27 degrees C	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-minute trains of electrical pulses ( alternate polarity , 2-ms duration ; 100 mA intensity ; 10 V drop between electrodes ; frequency 5 , 10 and 20 Hz ) applied to cultures kept at 27 degrees C , elicited a D - ( 3H ) aspartate outflow which was frequency related , ( Ca2 + ) 0 dependent , tetrodotoxin sensitive .
	manualset3
194520	13	415845	7	NULL	NULL	0	NULL	D - ( 3H ) aspartate outflow	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-minute trains of electrical pulses ( alternate polarity , 2-ms duration ; 100 mA intensity ; 10 V drop between electrodes ; frequency 5 , 10 and 20 Hz ) applied to cultures kept at 27 degrees C , elicited a D - ( 3H ) aspartate outflow which was frequency related , ( Ca2 + ) 0 dependent , tetrodotoxin sensitive .
	manualset3
194521	14	415845	7	NULL	NULL	0	NULL	( Ca2 + ) 0 dependent	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-minute trains of electrical pulses ( alternate polarity , 2-ms duration ; 100 mA intensity ; 10 V drop between electrodes ; frequency 5 , 10 and 20 Hz ) applied to cultures kept at 27 degrees C , elicited a D - ( 3H ) aspartate outflow which was frequency related , ( Ca2 + ) 0 dependent , tetrodotoxin sensitive .
	manualset3
194523	15	415845	7	NULL	NULL	0	NULL	tetrodotoxin sensitive	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-minute trains of electrical pulses ( alternate polarity , 2-ms duration ; 100 mA intensity ; 10 V drop between electrodes ; frequency 5 , 10 and 20 Hz ) applied to cultures kept at 27 degrees C , elicited a D - ( 3H ) aspartate outflow which was frequency related , ( Ca2 + ) 0 dependent , tetrodotoxin sensitive .
	manualset3
194528	1	415846	7	NULL	NULL	0	NULL	Two-stage laparoscopic biliopancreatic diversion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-stage laparoscopic biliopancreatic diversion with duodenal switch as treatment of high-risk super-obese patients : analysis of complications .
	manualset3
194529	2	415846	7	NULL	NULL	NULL	NULL	duodenal switch	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two-stage laparoscopic biliopancreatic diversion with duodenal switch as treatment of high-risk super-obese patients : analysis of complications .
	manualset3
194530	3	415846	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-stage laparoscopic biliopancreatic diversion with duodenal switch as treatment of high-risk super-obese patients : analysis of complications .
	manualset3
194531	4	415846	7	NULL	NULL	0	NULL	high-risk super-obese patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-stage laparoscopic biliopancreatic diversion with duodenal switch as treatment of high-risk super-obese patients : analysis of complications .
	manualset3
194532	5	415846	7	NULL	NULL	0	NULL	analysis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-stage laparoscopic biliopancreatic diversion with duodenal switch as treatment of high-risk super-obese patients : analysis of complications .
	manualset3
194533	6	415846	7	NULL	NULL	0	NULL	complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-stage laparoscopic biliopancreatic diversion with duodenal switch as treatment of high-risk super-obese patients : analysis of complications .
	manualset3
194534	1	415847	7	NULL	NULL	0	NULL	Two-thirds	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-thirds of the data set was used for the construction process and one-third was retained for validation .
	manualset3
194535	2	415847	7	NULL	NULL	0	NULL	data set	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-thirds of the data set was used for the construction process and one-third was retained for validation .
	manualset3
194536	3	415847	7	NULL	NULL	0	NULL	construction process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-thirds of the data set was used for the construction process and one-third was retained for validation .
	manualset3
194537	4	415847	7	NULL	NULL	0	NULL	one-third 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-thirds of the data set was used for the construction process and one-third was retained for validation .
	manualset3
194538	5	415847	7	NULL	NULL	0	NULL	validation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-thirds of the data set was used for the construction process and one-third was retained for validation .
	manualset3
194542	1	415848	7	NULL	NULL	0	NULL	Two-thirds	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-thirds of the patients had no complaints of nausea , and the majority of the remainder experienced only mild and transitory nausea .
	manualset3
194543	2	415848	7	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-thirds of the patients had no complaints of nausea , and the majority of the remainder experienced only mild and transitory nausea .
	manualset3
194544	3	415848	7	NULL	NULL	0	NULL	no complaints	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-thirds of the patients had no complaints of nausea , and the majority of the remainder experienced only mild and transitory nausea .
	manualset3
194545	4	415848	7	NULL	NULL	0	NULL	nausea	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-thirds of the patients had no complaints of nausea , and the majority of the remainder experienced only mild and transitory nausea .
	manualset3
194546	5	415848	7	NULL	NULL	0	NULL	majority	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-thirds of the patients had no complaints of nausea , and the majority of the remainder experienced only mild and transitory nausea .
	manualset3
194548	6	415848	7	NULL	NULL	0	NULL	remainder	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-thirds of the patients had no complaints of nausea , and the majority of the remainder experienced only mild and transitory nausea .
	manualset3
194549	7	415848	7	NULL	NULL	0	NULL	mild nausea	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-thirds of the patients had no complaints of nausea , and the majority of the remainder experienced only mild and transitory nausea .
	manualset3
194550	8	415848	7	NULL	NULL	0	NULL	transitory nausea	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-thirds of the patients had no complaints of nausea , and the majority of the remainder experienced only mild and transitory nausea .
	manualset3
194554	1	415849	7	NULL	NULL	0	NULL	purification 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After purification to near homogeneity , this enzyme was subjected to limited proteolysis and found to exhibit a high resistance to degradation and nicking .
	manualset3
194559	2	415849	7	NULL	NULL	NULL	NULL	homogeneity	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After purification to near homogeneity , this enzyme was subjected to limited proteolysis and found to exhibit a high resistance to degradation and nicking .
	manualset3
194560	3	415849	7	NULL	NULL	0	NULL	enzyme	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	After purification to near homogeneity , this enzyme was subjected to limited proteolysis and found to exhibit a high resistance to degradation and nicking .
	manualset3
194561	4	415849	7	NULL	NULL	0	NULL	limited proteolysis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After purification to near homogeneity , this enzyme was subjected to limited proteolysis and found to exhibit a high resistance to degradation and nicking .
	manualset3
194562	5	415849	7	NULL	NULL	0	NULL	 high resistance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After purification to near homogeneity , this enzyme was subjected to limited proteolysis and found to exhibit a high resistance to degradation and nicking .
	manualset3
194563	6	415849	7	NULL	NULL	0	NULL	degradation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After purification to near homogeneity , this enzyme was subjected to limited proteolysis and found to exhibit a high resistance to degradation and nicking .
	manualset3
194564	7	415849	7	NULL	NULL	0	NULL	nicking	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After purification to near homogeneity , this enzyme was subjected to limited proteolysis and found to exhibit a high resistance to degradation and nicking .
	manualset3
194568	1	415850	7	NULL	NULL	NULL	NULL	Two 14-3-3 binding motifs	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two 14-3-3 binding motifs are required for stable association of Forkhead transcription factor FOXO4 with 14-3-3 proteins and inhibition of DNA binding .
	manualset3
194570	2	415850	7	NULL	NULL	0	NULL	 stable association 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two 14-3-3 binding motifs are required for stable association of Forkhead transcription factor FOXO4 with 14-3-3 proteins and inhibition of DNA binding .
	manualset3
194571	3	415850	7	NULL	NULL	0	NULL	Forkhead transcription factor FOXO4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Two 14-3-3 binding motifs are required for stable association of Forkhead transcription factor FOXO4 with 14-3-3 proteins and inhibition of DNA binding .
	manualset3
194572	4	415850	7	NULL	NULL	0	NULL	14-3-3 proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two 14-3-3 binding motifs are required for stable association of Forkhead transcription factor FOXO4 with 14-3-3 proteins and inhibition of DNA binding .
	manualset3
194573	5	415850	7	NULL	NULL	0	NULL	inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two 14-3-3 binding motifs are required for stable association of Forkhead transcription factor FOXO4 with 14-3-3 proteins and inhibition of DNA binding .
	manualset3
194574	6	415850	7	NULL	NULL	0	NULL	DNA binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two 14-3-3 binding motifs are required for stable association of Forkhead transcription factor FOXO4 with 14-3-3 proteins and inhibition of DNA binding .
	manualset3
194575	1	415851	7	NULL	NULL	0	NULL	Two Atlantic coast species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two Atlantic coast species , Fundulus heteroclitus and Fundulus majalis , have unique derived acclimation responses .
	manualset3
194576	2	415851	7	NULL	NULL	0	NULL	Fundulus heteroclitus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two Atlantic coast species , Fundulus heteroclitus and Fundulus majalis , have unique derived acclimation responses .
	manualset3
194577	3	415851	7	NULL	NULL	0	NULL	Fundulus majalis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two Atlantic coast species , Fundulus heteroclitus and Fundulus majalis , have unique derived acclimation responses .
	manualset3
194578	4	415851	7	NULL	NULL	0	NULL	acclimation responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two Atlantic coast species , Fundulus heteroclitus and Fundulus majalis , have unique derived acclimation responses .
	manualset3
194632	1	415852	7	NULL	NULL	0	NULL	Two IRPs 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two IRPs ( IRP1 and IRP2 ) have been reported .
	manualset3
194633	2	415852	7	NULL	NULL	0	NULL	IRP1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Two IRPs ( IRP1 and IRP2 ) have been reported .
	manualset3
194635	3	415852	7	NULL	NULL	0	NULL	IRP2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Two IRPs ( IRP1 and IRP2 ) have been reported .
	manualset3
194637	1	415853	7	NULL	NULL	0	NULL	Two NF1 translocations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two NF1 translocations map within a 600-kilobase segment of 17q11 .2 .
	manualset3
194638	2	415853	7	NULL	NULL	0	NULL	600-kilobase segment	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Two NF1 translocations map within a 600-kilobase segment of 17q11 .2 .
	manualset3
194640	3	415853	7	NULL	NULL	0	NULL	17q11 .2 .	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Two NF1 translocations map within a 600-kilobase segment of 17q11 .2 .
	manualset3
194641	1	415854	7	NULL	NULL	0	NULL	Two P. berghei CQ resistant strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two P. berghei CQ resistant strains ( CQR6 and CQR30 ) were selected in vivo from the sensitive strain NK65 .
	manualset3
194642	2	415854	7	NULL	NULL	0	NULL	CQR6	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two P. berghei CQ resistant strains ( CQR6 and CQR30 ) were selected in vivo from the sensitive strain NK65 .
	manualset3
194643	3	415854	7	NULL	NULL	0	NULL	CQR30	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two P. berghei CQ resistant strains ( CQR6 and CQR30 ) were selected in vivo from the sensitive strain NK65 .
	manualset3
194644	4	415854	7	NULL	NULL	0	NULL	sensitive strain NK65	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two P. berghei CQ resistant strains ( CQR6 and CQR30 ) were selected in vivo from the sensitive strain NK65 .
	manualset3
194645	1	415855	7	NULL	NULL	0	NULL	Two SGBS kindreds	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two SGBS kindreds , with moderate expression of the condition , have been mapped to Xq27 .
	manualset3
194646	2	415855	7	NULL	NULL	0	NULL	moderate expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two SGBS kindreds , with moderate expression of the condition , have been mapped to Xq27 .
	manualset3
194647	3	415855	7	NULL	NULL	0	NULL	condition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two SGBS kindreds , with moderate expression of the condition , have been mapped to Xq27 .
	manualset3
194648	4	415855	7	NULL	NULL	0	NULL	Xq27	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Two SGBS kindreds , with moderate expression of the condition , have been mapped to Xq27 .
	manualset3
194649	1	415856	7	NULL	NULL	0	NULL	 radiation therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After radiation therapy to the lesion on the petrous bone , splenectomy was performed .
	manualset3
194650	2	415856	7	NULL	NULL	0	NULL	 lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After radiation therapy to the lesion on the petrous bone , splenectomy was performed .
	manualset3
194651	3	415856	7	NULL	NULL	0	NULL	 petrous bone	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After radiation therapy to the lesion on the petrous bone , splenectomy was performed .
	manualset3
194652	4	415856	7	NULL	NULL	0	NULL	 splenectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After radiation therapy to the lesion on the petrous bone , splenectomy was performed .
	manualset3
194653	1	415857	7	NULL	NULL	0	NULL	Two adult patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two adult patients ages 35 and 69 with constipation since birth underwent anorectal manometry .
	manualset3
194654	2	415857	7	NULL	NULL	0	NULL	ages 35	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Two adult patients ages 35 and 69 with constipation since birth underwent anorectal manometry .
	manualset3
194655	3	415857	7	NULL	NULL	0	NULL	ages 69	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Two adult patients ages 35 and 69 with constipation since birth underwent anorectal manometry .
	manualset3
194656	4	415857	7	NULL	NULL	0	NULL	constipation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two adult patients ages 35 and 69 with constipation since birth underwent anorectal manometry .
	manualset3
194657	5	415857	7	NULL	NULL	0	NULL	birth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two adult patients ages 35 and 69 with constipation since birth underwent anorectal manometry .
	manualset3
194658	6	415857	7	NULL	NULL	0	NULL	anorectal manometry	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Two adult patients ages 35 and 69 with constipation since birth underwent anorectal manometry .
	manualset3
194659	1	415858	7	NULL	NULL	0	NULL	Two alternatively spliced mouse paxillin cDNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Two alternatively spliced mouse paxillin cDNAs were cloned and in the process , a paxillin-related protein , Hic-5 , was also identified .
	manualset3
194660	2	415858	7	NULL	NULL	0	NULL	process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two alternatively spliced mouse paxillin cDNAs were cloned and in the process , a paxillin-related protein , Hic-5 , was also identified .
	manualset3
194661	3	415858	7	NULL	NULL	0	NULL	paxillin-related protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Two alternatively spliced mouse paxillin cDNAs were cloned and in the process , a paxillin-related protein , Hic-5 , was also identified .
	manualset3
194662	4	415858	7	NULL	NULL	0	NULL	Hic-5 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Two alternatively spliced mouse paxillin cDNAs were cloned and in the process , a paxillin-related protein , Hic-5 , was also identified .
	manualset3
194663	1	415859	7	NULL	NULL	NULL	NULL	Two anatomo-clinical cases	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two anatomo-clinical cases of downward gaze palsy and one case of upward gaze palsy are reported .
	manualset3
194664	2	415859	7	NULL	NULL	0	NULL	downward gaze palsy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two anatomo-clinical cases of downward gaze palsy and one case of upward gaze palsy are reported .
	manualset3
194665	3	415859	7	NULL	NULL	0	NULL	one case	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Two anatomo-clinical cases of downward gaze palsy and one case of upward gaze palsy are reported .
	manualset3
194666	4	415859	7	NULL	NULL	0	NULL	upward gaze palsy 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two anatomo-clinical cases of downward gaze palsy and one case of upward gaze palsy are reported .
	manualset3
194667	1	415860	7	NULL	NULL	0	NULL	Two and a half years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Two and a half years later , recurrence of HCC in the liver and its invasion to vena cava inferior ( IVC ) were found .
	manualset3
194668	2	415860	7	NULL	NULL	0	NULL	recurrence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two and a half years later , recurrence of HCC in the liver and its invasion to vena cava inferior ( IVC ) were found .
	manualset3
194669	3	415860	7	NULL	NULL	0	NULL	HCC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two and a half years later , recurrence of HCC in the liver and its invasion to vena cava inferior ( IVC ) were found .
	manualset3
194670	4	415860	7	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Two and a half years later , recurrence of HCC in the liver and its invasion to vena cava inferior ( IVC ) were found .
	manualset3
194671	5	415860	7	NULL	NULL	0	NULL	invasion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two and a half years later , recurrence of HCC in the liver and its invasion to vena cava inferior ( IVC ) were found .
	manualset3
194672	6	415860	7	NULL	NULL	0	NULL	vena cava inferior ( IVC )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Two and a half years later , recurrence of HCC in the liver and its invasion to vena cava inferior ( IVC ) were found .
	manualset3
194673	1	415861	7	NULL	NULL	0	NULL	Two approaches	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two approaches are presented for consideration in working with the stroke patient .
	manualset3
194674	2	415861	7	NULL	NULL	0	NULL	consideration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two approaches are presented for consideration in working with the stroke patient .
	manualset3
194675	3	415861	7	NULL	NULL	0	NULL	 working	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two approaches are presented for consideration in working with the stroke patient .
	manualset3
194676	4	415861	7	NULL	NULL	0	NULL	stroke patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Two approaches are presented for consideration in working with the stroke patient .
	manualset3
194677	1	415862	7	NULL	NULL	0	NULL	Two approaches	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two approaches investigated in the study were : ( 1 ) evaluation of vermistabilization of PSS and CD mixtures after 15 weeks in terms of fertilizer quality of the products and ; ( 2 ) growth and reproduction of Eisenia foetida up to 11 weeks in different vermireactors .
	manualset3
194678	2	415862	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two approaches investigated in the study were : ( 1 ) evaluation of vermistabilization of PSS and CD mixtures after 15 weeks in terms of fertilizer quality of the products and ; ( 2 ) growth and reproduction of Eisenia foetida up to 11 weeks in different vermireactors .
	manualset3
194679	3	415862	7	NULL	NULL	0	NULL	evaluation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two approaches investigated in the study were : ( 1 ) evaluation of vermistabilization of PSS and CD mixtures after 15 weeks in terms of fertilizer quality of the products and ; ( 2 ) growth and reproduction of Eisenia foetida up to 11 weeks in different vermireactors .
	manualset3
194680	4	415862	7	NULL	NULL	0	NULL	vermistabilization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two approaches investigated in the study were : ( 1 ) evaluation of vermistabilization of PSS and CD mixtures after 15 weeks in terms of fertilizer quality of the products and ; ( 2 ) growth and reproduction of Eisenia foetida up to 11 weeks in different vermireactors .
	manualset3
194681	5	415862	7	NULL	NULL	0	NULL	PSS	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two approaches investigated in the study were : ( 1 ) evaluation of vermistabilization of PSS and CD mixtures after 15 weeks in terms of fertilizer quality of the products and ; ( 2 ) growth and reproduction of Eisenia foetida up to 11 weeks in different vermireactors .
	manualset3
194682	6	415862	7	NULL	NULL	0	NULL	CD mixtures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two approaches investigated in the study were : ( 1 ) evaluation of vermistabilization of PSS and CD mixtures after 15 weeks in terms of fertilizer quality of the products and ; ( 2 ) growth and reproduction of Eisenia foetida up to 11 weeks in different vermireactors .
	manualset3
194683	7	415862	7	NULL	NULL	0	NULL	15 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Two approaches investigated in the study were : ( 1 ) evaluation of vermistabilization of PSS and CD mixtures after 15 weeks in terms of fertilizer quality of the products and ; ( 2 ) growth and reproduction of Eisenia foetida up to 11 weeks in different vermireactors .
	manualset3
194684	8	415862	7	NULL	NULL	0	NULL	terms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two approaches investigated in the study were : ( 1 ) evaluation of vermistabilization of PSS and CD mixtures after 15 weeks in terms of fertilizer quality of the products and ; ( 2 ) growth and reproduction of Eisenia foetida up to 11 weeks in different vermireactors .
	manualset3
194685	9	415862	7	NULL	NULL	NULL	NULL	fertilizer quality	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two approaches investigated in the study were : ( 1 ) evaluation of vermistabilization of PSS and CD mixtures after 15 weeks in terms of fertilizer quality of the products and ; ( 2 ) growth and reproduction of Eisenia foetida up to 11 weeks in different vermireactors .
	manualset3
194686	10	415862	7	NULL	NULL	0	NULL	products	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two approaches investigated in the study were : ( 1 ) evaluation of vermistabilization of PSS and CD mixtures after 15 weeks in terms of fertilizer quality of the products and ; ( 2 ) growth and reproduction of Eisenia foetida up to 11 weeks in different vermireactors .
	manualset3
194687	11	415862	7	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two approaches investigated in the study were : ( 1 ) evaluation of vermistabilization of PSS and CD mixtures after 15 weeks in terms of fertilizer quality of the products and ; ( 2 ) growth and reproduction of Eisenia foetida up to 11 weeks in different vermireactors .
	manualset3
194688	12	415862	7	NULL	NULL	0	NULL	reproduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two approaches investigated in the study were : ( 1 ) evaluation of vermistabilization of PSS and CD mixtures after 15 weeks in terms of fertilizer quality of the products and ; ( 2 ) growth and reproduction of Eisenia foetida up to 11 weeks in different vermireactors .
	manualset3
194689	13	415862	7	NULL	NULL	0	NULL	Eisenia foetida	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two approaches investigated in the study were : ( 1 ) evaluation of vermistabilization of PSS and CD mixtures after 15 weeks in terms of fertilizer quality of the products and ; ( 2 ) growth and reproduction of Eisenia foetida up to 11 weeks in different vermireactors .
	manualset3
194690	14	415862	7	NULL	NULL	0	NULL	11 weeks 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Two approaches investigated in the study were : ( 1 ) evaluation of vermistabilization of PSS and CD mixtures after 15 weeks in terms of fertilizer quality of the products and ; ( 2 ) growth and reproduction of Eisenia foetida up to 11 weeks in different vermireactors .
	manualset3
194691	15	415862	7	NULL	NULL	0	NULL	vermireactors 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Two approaches investigated in the study were : ( 1 ) evaluation of vermistabilization of PSS and CD mixtures after 15 weeks in terms of fertilizer quality of the products and ; ( 2 ) growth and reproduction of Eisenia foetida up to 11 weeks in different vermireactors .
	manualset3
194692	1	415863	7	NULL	NULL	0	NULL	Two articles	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Two articles noted the increase in the incidence of septic arthritis in children who are HIV-positive and another described a chlamydial-associated syndrome of arthritis and eye involvement .
	manualset3
194693	2	415863	7	NULL	NULL	0	NULL	 increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two articles noted the increase in the incidence of septic arthritis in children who are HIV-positive and another described a chlamydial-associated syndrome of arthritis and eye involvement .
	manualset3
194694	3	415863	7	NULL	NULL	0	NULL	 incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two articles noted the increase in the incidence of septic arthritis in children who are HIV-positive and another described a chlamydial-associated syndrome of arthritis and eye involvement .
	manualset3
194695	4	415863	7	NULL	NULL	0	NULL	septic arthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two articles noted the increase in the incidence of septic arthritis in children who are HIV-positive and another described a chlamydial-associated syndrome of arthritis and eye involvement .
	manualset3
194696	5	415863	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two articles noted the increase in the incidence of septic arthritis in children who are HIV-positive and another described a chlamydial-associated syndrome of arthritis and eye involvement .
	manualset3
194697	6	415863	7	NULL	NULL	0	NULL	HIV-positive	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two articles noted the increase in the incidence of septic arthritis in children who are HIV-positive and another described a chlamydial-associated syndrome of arthritis and eye involvement .
	manualset3
194698	7	415863	7	NULL	NULL	0	NULL	chlamydial-associated syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two articles noted the increase in the incidence of septic arthritis in children who are HIV-positive and another described a chlamydial-associated syndrome of arthritis and eye involvement .
	manualset3
194699	8	415863	7	NULL	NULL	0	NULL	arthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two articles noted the increase in the incidence of septic arthritis in children who are HIV-positive and another described a chlamydial-associated syndrome of arthritis and eye involvement .
	manualset3
194700	9	415863	7	NULL	NULL	0	NULL	eye involvement 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two articles noted the increase in the incidence of septic arthritis in children who are HIV-positive and another described a chlamydial-associated syndrome of arthritis and eye involvement .
	manualset3
194701	1	415864	7	NULL	NULL	0	NULL	reading	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After reading the entire novel , participants completed various memory tests in which they summarised the novel , provided associated information from cues , and answered specific questions .
	manualset3
194702	2	415864	7	NULL	NULL	0	NULL	entire novel	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	After reading the entire novel , participants completed various memory tests in which they summarised the novel , provided associated information from cues , and answered specific questions .
	manualset3
194703	3	415864	7	NULL	NULL	0	NULL	participants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	After reading the entire novel , participants completed various memory tests in which they summarised the novel , provided associated information from cues , and answered specific questions .
	manualset3
194704	4	415864	7	NULL	NULL	0	NULL	 memory tests 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After reading the entire novel , participants completed various memory tests in which they summarised the novel , provided associated information from cues , and answered specific questions .
	manualset3
194705	5	415864	7	NULL	NULL	0	NULL	novel	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	After reading the entire novel , participants completed various memory tests in which they summarised the novel , provided associated information from cues , and answered specific questions .
	manualset3
194706	6	415864	7	NULL	NULL	0	NULL	associated information	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After reading the entire novel , participants completed various memory tests in which they summarised the novel , provided associated information from cues , and answered specific questions .
	manualset3
194707	7	415864	7	NULL	NULL	0	NULL	cues	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After reading the entire novel , participants completed various memory tests in which they summarised the novel , provided associated information from cues , and answered specific questions .
	manualset3
194708	8	415864	7	NULL	NULL	0	NULL	questions 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	After reading the entire novel , participants completed various memory tests in which they summarised the novel , provided associated information from cues , and answered specific questions .
	manualset3
194709	1	415865	7	NULL	NULL	0	NULL	Two big challenges	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two big challenges of transplantation biology are controlling the reaction of the graft to the host after hematopoietic stem cell transplantation and preventing rejection of donor organs by the host .
	manualset3
194710	2	415865	7	NULL	NULL	0	NULL	transplantation biology 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Two big challenges of transplantation biology are controlling the reaction of the graft to the host after hematopoietic stem cell transplantation and preventing rejection of donor organs by the host .
	manualset3
194711	3	415865	7	NULL	NULL	0	NULL	reaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two big challenges of transplantation biology are controlling the reaction of the graft to the host after hematopoietic stem cell transplantation and preventing rejection of donor organs by the host .
	manualset3
194712	4	415865	7	NULL	NULL	0	NULL	 graft	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Two big challenges of transplantation biology are controlling the reaction of the graft to the host after hematopoietic stem cell transplantation and preventing rejection of donor organs by the host .
	manualset3
194713	5	415865	7	NULL	NULL	0	NULL	 host	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two big challenges of transplantation biology are controlling the reaction of the graft to the host after hematopoietic stem cell transplantation and preventing rejection of donor organs by the host .
	manualset3
194714	6	415865	7	NULL	NULL	0	NULL	hematopoietic stem cell transplantation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two big challenges of transplantation biology are controlling the reaction of the graft to the host after hematopoietic stem cell transplantation and preventing rejection of donor organs by the host .
	manualset3
194715	7	415865	7	NULL	NULL	0	NULL	 rejection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two big challenges of transplantation biology are controlling the reaction of the graft to the host after hematopoietic stem cell transplantation and preventing rejection of donor organs by the host .
	manualset3
194716	8	415865	7	NULL	NULL	0	NULL	donor organs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Two big challenges of transplantation biology are controlling the reaction of the graft to the host after hematopoietic stem cell transplantation and preventing rejection of donor organs by the host .
	manualset3
194717	9	415865	7	NULL	NULL	0	NULL	host	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two big challenges of transplantation biology are controlling the reaction of the graft to the host after hematopoietic stem cell transplantation and preventing rejection of donor organs by the host .
	manualset3
194785	1	415866	7	NULL	NULL	0	NULL	Two broiler trials	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two broiler trials were conducted to investigate the effect on post-mortem carcass and meat quality of NaHCO3 and KCl drinking water supplementation under thermoneutral and cyclic heat-stress climatic conditions .
	manualset3
194786	2	415866	7	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two broiler trials were conducted to investigate the effect on post-mortem carcass and meat quality of NaHCO3 and KCl drinking water supplementation under thermoneutral and cyclic heat-stress climatic conditions .
	manualset3
194787	3	415866	7	NULL	NULL	0	NULL	post-mortem carcass	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Two broiler trials were conducted to investigate the effect on post-mortem carcass and meat quality of NaHCO3 and KCl drinking water supplementation under thermoneutral and cyclic heat-stress climatic conditions .
	manualset3
194788	4	415866	7	NULL	NULL	0	NULL	meat quality	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two broiler trials were conducted to investigate the effect on post-mortem carcass and meat quality of NaHCO3 and KCl drinking water supplementation under thermoneutral and cyclic heat-stress climatic conditions .
	manualset3
194789	5	415866	7	NULL	NULL	0	NULL	NaHCO3	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two broiler trials were conducted to investigate the effect on post-mortem carcass and meat quality of NaHCO3 and KCl drinking water supplementation under thermoneutral and cyclic heat-stress climatic conditions .
	manualset3
194790	6	415866	7	NULL	NULL	0	NULL	KCl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two broiler trials were conducted to investigate the effect on post-mortem carcass and meat quality of NaHCO3 and KCl drinking water supplementation under thermoneutral and cyclic heat-stress climatic conditions .
	manualset3
194791	7	415866	7	NULL	NULL	NULL	NULL	drinking water supplementation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two broiler trials were conducted to investigate the effect on post-mortem carcass and meat quality of NaHCO3 and KCl drinking water supplementation under thermoneutral and cyclic heat-stress climatic conditions .
	manualset3
194792	8	415866	7	NULL	NULL	NULL	NULL	thermoneutral climatic conditions	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two broiler trials were conducted to investigate the effect on post-mortem carcass and meat quality of NaHCO3 and KCl drinking water supplementation under thermoneutral and cyclic heat-stress climatic conditions .
	manualset3
194793	9	415866	7	NULL	NULL	NULL	NULL	cyclic heat-stress climatic conditions	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two broiler trials were conducted to investigate the effect on post-mortem carcass and meat quality of NaHCO3 and KCl drinking water supplementation under thermoneutral and cyclic heat-stress climatic conditions .
	manualset3
194794	1	415867	7	NULL	NULL	0	NULL	Two brothers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two brothers , including one with C-monosomy , died with hypoplastic anemia and another brother died with acute myelocytic leukemia .
	manualset3
194795	2	415867	7	NULL	NULL	0	NULL	one	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two brothers , including one with C-monosomy , died with hypoplastic anemia and another brother died with acute myelocytic leukemia .
	manualset3
194796	3	415867	7	NULL	NULL	0	NULL	C-monosomy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two brothers , including one with C-monosomy , died with hypoplastic anemia and another brother died with acute myelocytic leukemia .
	manualset3
194797	4	415867	7	NULL	NULL	NULL	NULL	 hypoplastic anemia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two brothers , including one with C-monosomy , died with hypoplastic anemia and another brother died with acute myelocytic leukemia .
	manualset3
194798	5	415867	7	NULL	NULL	NULL	NULL	 brother	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two brothers , including one with C-monosomy , died with hypoplastic anemia and another brother died with acute myelocytic leukemia .
	manualset3
194799	6	415867	7	NULL	NULL	0	NULL	acute myelocytic leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two brothers , including one with C-monosomy , died with hypoplastic anemia and another brother died with acute myelocytic leukemia .
	manualset3
194800	1	415868	7	NULL	NULL	0	NULL	Two brothers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two brothers with pathological medial plicae are described in whom the condition was mistaken for arthritis .
	manualset3
194801	2	415868	7	NULL	NULL	0	NULL	pathological medial plicae	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two brothers with pathological medial plicae are described in whom the condition was mistaken for arthritis .
	manualset3
194802	3	415868	7	NULL	NULL	NULL	NULL	condition	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two brothers with pathological medial plicae are described in whom the condition was mistaken for arthritis .
	manualset3
194803	4	415868	7	NULL	NULL	0	NULL	arthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two brothers with pathological medial plicae are described in whom the condition was mistaken for arthritis .
	manualset3
194804	1	415869	7	NULL	NULL	0	NULL	Two buffers 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two buffers of different pH created a junction to trap the sample molecules at their isoelectric points and resulted in over 1000-fold preconcentration for myoglobin within 30 min .
	manualset3
194805	2	415869	7	NULL	NULL	0	NULL	different pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two buffers of different pH created a junction to trap the sample molecules at their isoelectric points and resulted in over 1000-fold preconcentration for myoglobin within 30 min .
	manualset3
194806	3	415869	7	NULL	NULL	0	NULL	junction	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two buffers of different pH created a junction to trap the sample molecules at their isoelectric points and resulted in over 1000-fold preconcentration for myoglobin within 30 min .
	manualset3
194807	4	415869	7	NULL	NULL	0	NULL	sample molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Two buffers of different pH created a junction to trap the sample molecules at their isoelectric points and resulted in over 1000-fold preconcentration for myoglobin within 30 min .
	manualset3
194808	5	415869	7	NULL	NULL	0	NULL	isoelectric points	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two buffers of different pH created a junction to trap the sample molecules at their isoelectric points and resulted in over 1000-fold preconcentration for myoglobin within 30 min .
	manualset3
194809	6	415869	7	NULL	NULL	0	NULL	1000-fold preconcentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two buffers of different pH created a junction to trap the sample molecules at their isoelectric points and resulted in over 1000-fold preconcentration for myoglobin within 30 min .
	manualset3
194810	7	415869	7	NULL	NULL	0	NULL	myoglobin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Two buffers of different pH created a junction to trap the sample molecules at their isoelectric points and resulted in over 1000-fold preconcentration for myoglobin within 30 min .
	manualset3
194811	8	415869	7	NULL	NULL	0	NULL	30 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Two buffers of different pH created a junction to trap the sample molecules at their isoelectric points and resulted in over 1000-fold preconcentration for myoglobin within 30 min .
	manualset3
194812	1	415870	7	NULL	NULL	0	NULL	Two cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases ( 0.6 % ; 95 % confidence limits 0.1-2 .2 % ) of fetal chromosome abnormality were found : one case of Klinefelter 's syndrome and one case of de novo translocation .
	manualset3
194813	2	415870	7	NULL	NULL	0	NULL	 0.6 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases ( 0.6 % ; 95 % confidence limits 0.1-2 .2 % ) of fetal chromosome abnormality were found : one case of Klinefelter 's syndrome and one case of de novo translocation .
	manualset3
194814	3	415870	7	NULL	NULL	0	NULL	95 % confidence limits	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases ( 0.6 % ; 95 % confidence limits 0.1-2 .2 % ) of fetal chromosome abnormality were found : one case of Klinefelter 's syndrome and one case of de novo translocation .
	manualset3
194815	4	415870	7	NULL	NULL	0	NULL	0.1-2 .2 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases ( 0.6 % ; 95 % confidence limits 0.1-2 .2 % ) of fetal chromosome abnormality were found : one case of Klinefelter 's syndrome and one case of de novo translocation .
	manualset3
194816	5	415870	7	NULL	NULL	0	NULL	fetal chromosome abnormality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases ( 0.6 % ; 95 % confidence limits 0.1-2 .2 % ) of fetal chromosome abnormality were found : one case of Klinefelter 's syndrome and one case of de novo translocation .
	manualset3
194817	6	415870	7	NULL	NULL	0	NULL	one case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases ( 0.6 % ; 95 % confidence limits 0.1-2 .2 % ) of fetal chromosome abnormality were found : one case of Klinefelter 's syndrome and one case of de novo translocation .
	manualset3
194818	7	415870	7	NULL	NULL	0	NULL	Klinefelter 's syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases ( 0.6 % ; 95 % confidence limits 0.1-2 .2 % ) of fetal chromosome abnormality were found : one case of Klinefelter 's syndrome and one case of de novo translocation .
	manualset3
194819	8	415870	7	NULL	NULL	0	NULL	one case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases ( 0.6 % ; 95 % confidence limits 0.1-2 .2 % ) of fetal chromosome abnormality were found : one case of Klinefelter 's syndrome and one case of de novo translocation .
	manualset3
194820	9	415870	7	NULL	NULL	0	NULL	de novo translocation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases ( 0.6 % ; 95 % confidence limits 0.1-2 .2 % ) of fetal chromosome abnormality were found : one case of Klinefelter 's syndrome and one case of de novo translocation .
	manualset3
194891	1	415871	7	NULL	NULL	NULL	NULL	Two cases	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two cases and literature review ) .
	manualset3
194892	2	415871	7	NULL	NULL	0	NULL	 literature review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases and literature review ) .
	manualset3
194893	1	415872	7	NULL	NULL	NULL	NULL	Two cases	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two cases exhibiting great variability of diaphragmatic CT appearance are reported .
	manualset3
194894	2	415872	7	NULL	NULL	0	NULL	great variability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases exhibiting great variability of diaphragmatic CT appearance are reported .
	manualset3
194895	3	415872	7	NULL	NULL	0	NULL	diaphragmatic CT appearance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases exhibiting great variability of diaphragmatic CT appearance are reported .
	manualset3
194904	1	415873	7	NULL	NULL	0	NULL	Two cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of Hemophilus influenzae septic arthritis are reported , one in a rheumatoid patient and the other in a healthy young woman after meningitis .
	manualset3
194906	2	415873	7	NULL	NULL	0	NULL	Hemophilus influenzae septic arthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of Hemophilus influenzae septic arthritis are reported , one in a rheumatoid patient and the other in a healthy young woman after meningitis .
	manualset3
194908	3	415873	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of Hemophilus influenzae septic arthritis are reported , one in a rheumatoid patient and the other in a healthy young woman after meningitis .
	manualset3
194911	4	415873	7	NULL	NULL	0	NULL	rheumatoid patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of Hemophilus influenzae septic arthritis are reported , one in a rheumatoid patient and the other in a healthy young woman after meningitis .
	manualset3
194912	5	415873	7	NULL	NULL	0	NULL	healthy young woman	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of Hemophilus influenzae septic arthritis are reported , one in a rheumatoid patient and the other in a healthy young woman after meningitis .
	manualset3
194913	6	415873	7	NULL	NULL	0	NULL	meningitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of Hemophilus influenzae septic arthritis are reported , one in a rheumatoid patient and the other in a healthy young woman after meningitis .
	manualset3
194914	1	415874	7	NULL	NULL	0	NULL	recurrence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After recurrence of chylous ascites , conservative treatment for three months including parenteral nutrition and low-fat diet under continuous peritoneal drainage led finally to success .
	manualset3
194915	2	415874	7	NULL	NULL	0	NULL	chylous ascites	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	After recurrence of chylous ascites , conservative treatment for three months including parenteral nutrition and low-fat diet under continuous peritoneal drainage led finally to success .
	manualset3
194916	3	415874	7	NULL	NULL	0	NULL	conservative treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After recurrence of chylous ascites , conservative treatment for three months including parenteral nutrition and low-fat diet under continuous peritoneal drainage led finally to success .
	manualset3
194917	4	415874	7	NULL	NULL	0	NULL	three months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After recurrence of chylous ascites , conservative treatment for three months including parenteral nutrition and low-fat diet under continuous peritoneal drainage led finally to success .
	manualset3
194918	5	415874	7	NULL	NULL	0	NULL	parenteral nutrition	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	After recurrence of chylous ascites , conservative treatment for three months including parenteral nutrition and low-fat diet under continuous peritoneal drainage led finally to success .
	manualset3
194919	6	415874	7	NULL	NULL	0	NULL	low-fat diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	After recurrence of chylous ascites , conservative treatment for three months including parenteral nutrition and low-fat diet under continuous peritoneal drainage led finally to success .
	manualset3
194920	7	415874	7	NULL	NULL	NULL	NULL	continuous peritoneal drainage	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After recurrence of chylous ascites , conservative treatment for three months including parenteral nutrition and low-fat diet under continuous peritoneal drainage led finally to success .
	manualset3
196346	8	415874	7	NULL	NULL	0	NULL	success	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After recurrence of chylous ascites , conservative treatment for three months including parenteral nutrition and low-fat diet under continuous peritoneal drainage led finally to success .
	manualset3
194921	1	415875	7	NULL	NULL	0	NULL	Two cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of Ramsey-Hunt Syndrome are reported , one of which presented features of the Guillain-Barr Syndrome .
	manualset3
194922	2	415875	7	NULL	NULL	0	NULL	Ramsey-Hunt Syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of Ramsey-Hunt Syndrome are reported , one of which presented features of the Guillain-Barr Syndrome .
	manualset3
194923	3	415875	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of Ramsey-Hunt Syndrome are reported , one of which presented features of the Guillain-Barr Syndrome .
	manualset3
194924	4	415875	7	NULL	NULL	0	NULL	Guillain-Barr Syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of Ramsey-Hunt Syndrome are reported , one of which presented features of the Guillain-Barr Syndrome .
	manualset3
194925	1	415876	7	NULL	NULL	0	NULL	Two cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of atopic dermatitis-like conditions induced in psoriasis patients treated with infliximab .
	manualset3
194926	2	415876	7	NULL	NULL	0	NULL	atopic dermatitis-like conditions	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of atopic dermatitis-like conditions induced in psoriasis patients treated with infliximab .
	manualset3
194927	3	415876	7	NULL	NULL	0	NULL	psoriasis patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of atopic dermatitis-like conditions induced in psoriasis patients treated with infliximab .
	manualset3
194928	4	415876	7	NULL	NULL	0	NULL	infliximab	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of atopic dermatitis-like conditions induced in psoriasis patients treated with infliximab .
	manualset3
194929	1	415877	7	NULL	NULL	0	NULL	Two cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of metastatic renal tumor are reported , one in a 78-year-old male who had undergone total gastrectomy for gastric carcinoma , and the other in a 45-year-old female who had undergone hysterectomy for cervical carcinoma of the uterus .
	manualset3
194930	2	415877	7	NULL	NULL	0	NULL	metastatic renal tumor	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of metastatic renal tumor are reported , one in a 78-year-old male who had undergone total gastrectomy for gastric carcinoma , and the other in a 45-year-old female who had undergone hysterectomy for cervical carcinoma of the uterus .
	manualset3
194932	3	415877	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of metastatic renal tumor are reported , one in a 78-year-old male who had undergone total gastrectomy for gastric carcinoma , and the other in a 45-year-old female who had undergone hysterectomy for cervical carcinoma of the uterus .
	manualset3
194935	4	415877	7	NULL	NULL	0	NULL	78-year-old male	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of metastatic renal tumor are reported , one in a 78-year-old male who had undergone total gastrectomy for gastric carcinoma , and the other in a 45-year-old female who had undergone hysterectomy for cervical carcinoma of the uterus .
	manualset3
194938	5	415877	7	NULL	NULL	0	NULL	total gastrectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of metastatic renal tumor are reported , one in a 78-year-old male who had undergone total gastrectomy for gastric carcinoma , and the other in a 45-year-old female who had undergone hysterectomy for cervical carcinoma of the uterus .
	manualset3
194940	6	415877	7	NULL	NULL	0	NULL	gastric carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of metastatic renal tumor are reported , one in a 78-year-old male who had undergone total gastrectomy for gastric carcinoma , and the other in a 45-year-old female who had undergone hysterectomy for cervical carcinoma of the uterus .
	manualset3
194942	7	415877	7	NULL	NULL	0	NULL	45-year-old female	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of metastatic renal tumor are reported , one in a 78-year-old male who had undergone total gastrectomy for gastric carcinoma , and the other in a 45-year-old female who had undergone hysterectomy for cervical carcinoma of the uterus .
	manualset3
194943	8	415877	7	NULL	NULL	0	NULL	hysterectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of metastatic renal tumor are reported , one in a 78-year-old male who had undergone total gastrectomy for gastric carcinoma , and the other in a 45-year-old female who had undergone hysterectomy for cervical carcinoma of the uterus .
	manualset3
194944	9	415877	7	NULL	NULL	0	NULL	cervical carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of metastatic renal tumor are reported , one in a 78-year-old male who had undergone total gastrectomy for gastric carcinoma , and the other in a 45-year-old female who had undergone hysterectomy for cervical carcinoma of the uterus .
	manualset3
194945	10	415877	7	NULL	NULL	0	NULL	uterus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of metastatic renal tumor are reported , one in a 78-year-old male who had undergone total gastrectomy for gastric carcinoma , and the other in a 45-year-old female who had undergone hysterectomy for cervical carcinoma of the uterus .
	manualset3
194950	1	415878	7	NULL	NULL	0	NULL	Two cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of neurofibromatosis and intracranial arterial occlusive disease are reported .
	manualset3
194953	2	415878	7	NULL	NULL	0	NULL	neurofibromatosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of neurofibromatosis and intracranial arterial occlusive disease are reported .
	manualset3
194954	3	415878	7	NULL	NULL	0	NULL	intracranial arterial occlusive disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of neurofibromatosis and intracranial arterial occlusive disease are reported .
	manualset3
194955	1	415879	7	NULL	NULL	0	NULL	Two cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of smoke inhalation injury are reported with a brief review of the pertinent literature .
	manualset3
194956	2	415879	7	NULL	NULL	0	NULL	smoke inhalation injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of smoke inhalation injury are reported with a brief review of the pertinent literature .
	manualset3
194958	3	415879	7	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of smoke inhalation injury are reported with a brief review of the pertinent literature .
	manualset3
194960	4	415879	7	NULL	NULL	0	NULL	pertinent literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of smoke inhalation injury are reported with a brief review of the pertinent literature .
	manualset3
194963	1	415880	7	NULL	NULL	0	NULL	Two children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two children died of sepsis and CNS damage or MOF , and one patient died during transplantation because of cardiac failure .
	manualset3
194964	2	415880	7	NULL	NULL	0	NULL	sepsis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two children died of sepsis and CNS damage or MOF , and one patient died during transplantation because of cardiac failure .
	manualset3
194966	3	415880	7	NULL	NULL	0	NULL	CNS damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two children died of sepsis and CNS damage or MOF , and one patient died during transplantation because of cardiac failure .
	manualset3
194978	4	415880	7	NULL	NULL	0	NULL	MOF	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two children died of sepsis and CNS damage or MOF , and one patient died during transplantation because of cardiac failure .
	manualset3
194980	5	415880	7	NULL	NULL	0	NULL	one patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Two children died of sepsis and CNS damage or MOF , and one patient died during transplantation because of cardiac failure .
	manualset3
194981	6	415880	7	NULL	NULL	0	NULL	transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Two children died of sepsis and CNS damage or MOF , and one patient died during transplantation because of cardiac failure .
	manualset3
194983	7	415880	7	NULL	NULL	0	NULL	cardiac failure	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two children died of sepsis and CNS damage or MOF , and one patient died during transplantation because of cardiac failure .
	manualset3
194986	1	415881	7	NULL	NULL	0	NULL	Two chromium-resistant bacterial strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two chromium-resistant bacterial strains , CrT-1 and CrT-13 , tolerant up to 40 mg K2CrO4 ml ( -1 ) on nutrient agar , 25 mg ml ( -1 ) in nutrient broth , and up to 10 mg ml ( -1 ) in acetate-minimal media , were identified as Ochrobactrum intermedium and Brevibacterium sp. , respectively , on the basis of 16S rRNA gene sequencing .
	manualset3
194987	2	415881	7	NULL	NULL	0	NULL	 CrT-1	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two chromium-resistant bacterial strains , CrT-1 and CrT-13 , tolerant up to 40 mg K2CrO4 ml ( -1 ) on nutrient agar , 25 mg ml ( -1 ) in nutrient broth , and up to 10 mg ml ( -1 ) in acetate-minimal media , were identified as Ochrobactrum intermedium and Brevibacterium sp. , respectively , on the basis of 16S rRNA gene sequencing .
	manualset3
194988	3	415881	7	NULL	NULL	0	NULL	CrT-13	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two chromium-resistant bacterial strains , CrT-1 and CrT-13 , tolerant up to 40 mg K2CrO4 ml ( -1 ) on nutrient agar , 25 mg ml ( -1 ) in nutrient broth , and up to 10 mg ml ( -1 ) in acetate-minimal media , were identified as Ochrobactrum intermedium and Brevibacterium sp. , respectively , on the basis of 16S rRNA gene sequencing .
	manualset3
194990	4	415881	7	NULL	NULL	0	NULL	 40 mg	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two chromium-resistant bacterial strains , CrT-1 and CrT-13 , tolerant up to 40 mg K2CrO4 ml ( -1 ) on nutrient agar , 25 mg ml ( -1 ) in nutrient broth , and up to 10 mg ml ( -1 ) in acetate-minimal media , were identified as Ochrobactrum intermedium and Brevibacterium sp. , respectively , on the basis of 16S rRNA gene sequencing .
	manualset3
194991	5	415881	7	NULL	NULL	0	NULL	K2CrO4 ml ( -1 ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two chromium-resistant bacterial strains , CrT-1 and CrT-13 , tolerant up to 40 mg K2CrO4 ml ( -1 ) on nutrient agar , 25 mg ml ( -1 ) in nutrient broth , and up to 10 mg ml ( -1 ) in acetate-minimal media , were identified as Ochrobactrum intermedium and Brevibacterium sp. , respectively , on the basis of 16S rRNA gene sequencing .
	manualset3
194993	6	415881	7	NULL	NULL	0	NULL	nutrient agar	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two chromium-resistant bacterial strains , CrT-1 and CrT-13 , tolerant up to 40 mg K2CrO4 ml ( -1 ) on nutrient agar , 25 mg ml ( -1 ) in nutrient broth , and up to 10 mg ml ( -1 ) in acetate-minimal media , were identified as Ochrobactrum intermedium and Brevibacterium sp. , respectively , on the basis of 16S rRNA gene sequencing .
	manualset3
194995	7	415881	7	NULL	NULL	0	NULL	25 mg ml ( -1 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two chromium-resistant bacterial strains , CrT-1 and CrT-13 , tolerant up to 40 mg K2CrO4 ml ( -1 ) on nutrient agar , 25 mg ml ( -1 ) in nutrient broth , and up to 10 mg ml ( -1 ) in acetate-minimal media , were identified as Ochrobactrum intermedium and Brevibacterium sp. , respectively , on the basis of 16S rRNA gene sequencing .
	manualset3
194998	8	415881	7	NULL	NULL	0	NULL	nutrient broth	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two chromium-resistant bacterial strains , CrT-1 and CrT-13 , tolerant up to 40 mg K2CrO4 ml ( -1 ) on nutrient agar , 25 mg ml ( -1 ) in nutrient broth , and up to 10 mg ml ( -1 ) in acetate-minimal media , were identified as Ochrobactrum intermedium and Brevibacterium sp. , respectively , on the basis of 16S rRNA gene sequencing .
	manualset3
194999	9	415881	7	NULL	NULL	0	NULL	10 mg ml ( -1 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two chromium-resistant bacterial strains , CrT-1 and CrT-13 , tolerant up to 40 mg K2CrO4 ml ( -1 ) on nutrient agar , 25 mg ml ( -1 ) in nutrient broth , and up to 10 mg ml ( -1 ) in acetate-minimal media , were identified as Ochrobactrum intermedium and Brevibacterium sp. , respectively , on the basis of 16S rRNA gene sequencing .
	manualset3
195000	10	415881	7	NULL	NULL	0	NULL	acetate-minimal media 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two chromium-resistant bacterial strains , CrT-1 and CrT-13 , tolerant up to 40 mg K2CrO4 ml ( -1 ) on nutrient agar , 25 mg ml ( -1 ) in nutrient broth , and up to 10 mg ml ( -1 ) in acetate-minimal media , were identified as Ochrobactrum intermedium and Brevibacterium sp. , respectively , on the basis of 16S rRNA gene sequencing .
	manualset3
195001	11	415881	7	NULL	NULL	0	NULL	Ochrobactrum intermedium	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two chromium-resistant bacterial strains , CrT-1 and CrT-13 , tolerant up to 40 mg K2CrO4 ml ( -1 ) on nutrient agar , 25 mg ml ( -1 ) in nutrient broth , and up to 10 mg ml ( -1 ) in acetate-minimal media , were identified as Ochrobactrum intermedium and Brevibacterium sp. , respectively , on the basis of 16S rRNA gene sequencing .
	manualset3
195002	12	415881	7	NULL	NULL	0	NULL	Brevibacterium sp. ,	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two chromium-resistant bacterial strains , CrT-1 and CrT-13 , tolerant up to 40 mg K2CrO4 ml ( -1 ) on nutrient agar , 25 mg ml ( -1 ) in nutrient broth , and up to 10 mg ml ( -1 ) in acetate-minimal media , were identified as Ochrobactrum intermedium and Brevibacterium sp. , respectively , on the basis of 16S rRNA gene sequencing .
	manualset3
195003	13	415881	7	NULL	NULL	0	NULL	basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two chromium-resistant bacterial strains , CrT-1 and CrT-13 , tolerant up to 40 mg K2CrO4 ml ( -1 ) on nutrient agar , 25 mg ml ( -1 ) in nutrient broth , and up to 10 mg ml ( -1 ) in acetate-minimal media , were identified as Ochrobactrum intermedium and Brevibacterium sp. , respectively , on the basis of 16S rRNA gene sequencing .
	manualset3
195004	14	415881	7	NULL	NULL	0	NULL	16S rRNA gene sequencing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two chromium-resistant bacterial strains , CrT-1 and CrT-13 , tolerant up to 40 mg K2CrO4 ml ( -1 ) on nutrient agar , 25 mg ml ( -1 ) in nutrient broth , and up to 10 mg ml ( -1 ) in acetate-minimal media , were identified as Ochrobactrum intermedium and Brevibacterium sp. , respectively , on the basis of 16S rRNA gene sequencing .
	manualset3
195007	1	415882	7	NULL	NULL	0	NULL	Two classic animal behavior despair tests	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Two classic animal behavior despair tests -- the Forced Swimming Test ( FST ) and the Tail Suspension Test ( TST ) were used to evaluate the antidepressant activity of liquiritin and isoliquiritin from Glycyrrhiza uralensis in mice .
	manualset3
195009	2	415882	7	NULL	NULL	0	NULL	the Forced Swimming Test ( FST ) 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Two classic animal behavior despair tests -- the Forced Swimming Test ( FST ) and the Tail Suspension Test ( TST ) were used to evaluate the antidepressant activity of liquiritin and isoliquiritin from Glycyrrhiza uralensis in mice .
	manualset3
195012	3	415882	7	NULL	NULL	0	NULL	Tail Suspension Test ( TST ) 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Two classic animal behavior despair tests -- the Forced Swimming Test ( FST ) and the Tail Suspension Test ( TST ) were used to evaluate the antidepressant activity of liquiritin and isoliquiritin from Glycyrrhiza uralensis in mice .
	manualset3
195013	4	415882	7	NULL	NULL	0	NULL	antidepressant activity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two classic animal behavior despair tests -- the Forced Swimming Test ( FST ) and the Tail Suspension Test ( TST ) were used to evaluate the antidepressant activity of liquiritin and isoliquiritin from Glycyrrhiza uralensis in mice .
	manualset3
195014	5	415882	7	NULL	NULL	0	NULL	 liquiritin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two classic animal behavior despair tests -- the Forced Swimming Test ( FST ) and the Tail Suspension Test ( TST ) were used to evaluate the antidepressant activity of liquiritin and isoliquiritin from Glycyrrhiza uralensis in mice .
	manualset3
195015	6	415882	7	NULL	NULL	0	NULL	isoliquiritin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two classic animal behavior despair tests -- the Forced Swimming Test ( FST ) and the Tail Suspension Test ( TST ) were used to evaluate the antidepressant activity of liquiritin and isoliquiritin from Glycyrrhiza uralensis in mice .
	manualset3
195016	7	415882	7	NULL	NULL	0	NULL	Glycyrrhiza uralensis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two classic animal behavior despair tests -- the Forced Swimming Test ( FST ) and the Tail Suspension Test ( TST ) were used to evaluate the antidepressant activity of liquiritin and isoliquiritin from Glycyrrhiza uralensis in mice .
	manualset3
195017	8	415882	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two classic animal behavior despair tests -- the Forced Swimming Test ( FST ) and the Tail Suspension Test ( TST ) were used to evaluate the antidepressant activity of liquiritin and isoliquiritin from Glycyrrhiza uralensis in mice .
	manualset3
195023	1	415883	7	NULL	NULL	0	NULL	alternative explanations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After refuting alternative explanations for this pattern , we conclude that marker mutation rate indeed has had a biasing effect on published Q ( ST ) - F ( ST ) comparisons .
	manualset3
195024	2	415883	7	NULL	NULL	0	NULL	pattern	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After refuting alternative explanations for this pattern , we conclude that marker mutation rate indeed has had a biasing effect on published Q ( ST ) - F ( ST ) comparisons .
	manualset3
195025	3	415883	7	NULL	NULL	0	NULL	marker mutation rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After refuting alternative explanations for this pattern , we conclude that marker mutation rate indeed has had a biasing effect on published Q ( ST ) - F ( ST ) comparisons .
	manualset3
195026	4	415883	7	NULL	NULL	0	NULL	biasing effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After refuting alternative explanations for this pattern , we conclude that marker mutation rate indeed has had a biasing effect on published Q ( ST ) - F ( ST ) comparisons .
	manualset3
195027	5	415883	7	NULL	NULL	0	NULL	published Q ( ST ) - F ( ST ) comparisons	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	After refuting alternative explanations for this pattern , we conclude that marker mutation rate indeed has had a biasing effect on published Q ( ST ) - F ( ST ) comparisons .
	manualset3
195028	1	415884	7	NULL	NULL	0	NULL	Two clinical cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two clinical cases of traumatic cataract , occurring in young patients , were analyzed .
	manualset3
195029	2	415884	7	NULL	NULL	0	NULL	traumatic cataract	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two clinical cases of traumatic cataract , occurring in young patients , were analyzed .
	manualset3
195030	3	415884	7	NULL	NULL	0	NULL	young patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two clinical cases of traumatic cataract , occurring in young patients , were analyzed .
	manualset3
195041	1	415885	7	NULL	NULL	0	NULL	Two cohorts	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cohorts were analyzed : one receiving MAGE-3 protein alone , and one receiving MAGE-3 protein with adjuvant AS02B .
	manualset3
195043	2	415885	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cohorts were analyzed : one receiving MAGE-3 protein alone , and one receiving MAGE-3 protein with adjuvant AS02B .
	manualset3
195044	3	415885	7	NULL	NULL	0	NULL	MAGE-3 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cohorts were analyzed : one receiving MAGE-3 protein alone , and one receiving MAGE-3 protein with adjuvant AS02B .
	manualset3
195045	4	415885	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cohorts were analyzed : one receiving MAGE-3 protein alone , and one receiving MAGE-3 protein with adjuvant AS02B .
	manualset3
195047	5	415885	7	NULL	NULL	0	NULL	MAGE-3 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cohorts were analyzed : one receiving MAGE-3 protein alone , and one receiving MAGE-3 protein with adjuvant AS02B .
	manualset3
195049	6	415885	7	NULL	NULL	0	NULL	adjuvant AS02B	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cohorts were analyzed : one receiving MAGE-3 protein alone , and one receiving MAGE-3 protein with adjuvant AS02B .
	manualset3
195050	1	415886	7	NULL	NULL	0	NULL	Two days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Two days later , conscious rats were infused with whole blood to expand blood volume .
	manualset3
195051	2	415886	7	NULL	NULL	0	NULL	 conscious rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two days later , conscious rats were infused with whole blood to expand blood volume .
	manualset3
195052	3	415886	7	NULL	NULL	0	NULL	whole blood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Two days later , conscious rats were infused with whole blood to expand blood volume .
	manualset3
195053	4	415886	7	NULL	NULL	0	NULL	blood volume 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two days later , conscious rats were infused with whole blood to expand blood volume .
	manualset3
195054	1	415887	7	NULL	NULL	0	NULL	Two demographic factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two demographic factors , Udmurt ethnicity and unmarried marital status , were significantly associated with both recurrent and chronic course of depression .
	manualset3
195055	2	415887	7	NULL	NULL	0	NULL	Udmurt ethnicity	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two demographic factors , Udmurt ethnicity and unmarried marital status , were significantly associated with both recurrent and chronic course of depression .
	manualset3
195056	3	415887	7	NULL	NULL	0	NULL	unmarried marital status	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two demographic factors , Udmurt ethnicity and unmarried marital status , were significantly associated with both recurrent and chronic course of depression .
	manualset3
195057	4	415887	7	NULL	NULL	0	NULL	 recurrent course	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Two demographic factors , Udmurt ethnicity and unmarried marital status , were significantly associated with both recurrent and chronic course of depression .
	manualset3
195059	5	415887	7	NULL	NULL	0	NULL	chronic course	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Two demographic factors , Udmurt ethnicity and unmarried marital status , were significantly associated with both recurrent and chronic course of depression .
	manualset3
195061	6	415887	7	NULL	NULL	0	NULL	depression	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two demographic factors , Udmurt ethnicity and unmarried marital status , were significantly associated with both recurrent and chronic course of depression .
	manualset3
195089	1	415888	7	NULL	NULL	0	NULL	Two dichromats	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two dichromats and two anomalous trichromats did not show clear evidence of LWS vs MWS cone antagonism .
	manualset3
195090	2	415888	7	NULL	NULL	0	NULL	two anomalous trichromats	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two dichromats and two anomalous trichromats did not show clear evidence of LWS vs MWS cone antagonism .
	manualset3
195092	3	415888	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two dichromats and two anomalous trichromats did not show clear evidence of LWS vs MWS cone antagonism .
	manualset3
195094	4	415888	7	NULL	NULL	0	NULL	LWS cone antagonism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two dichromats and two anomalous trichromats did not show clear evidence of LWS vs MWS cone antagonism .
	manualset3
195096	5	415888	7	NULL	NULL	0	NULL	MWS cone antagonism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two dichromats and two anomalous trichromats did not show clear evidence of LWS vs MWS cone antagonism .
	manualset3
195098	1	415889	7	NULL	NULL	0	NULL	Two different methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two different methods were compared in the assessment of depressive symptomatology improvement : live naturalistic ( N ) performed by the patient 's therapist , and from videotape record of structured clinical interview ( VSI ) assessed by an independent rater out of five psychiatrists .
	manualset3
195099	2	415889	7	NULL	NULL	0	NULL	assessment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Two different methods were compared in the assessment of depressive symptomatology improvement : live naturalistic ( N ) performed by the patient 's therapist , and from videotape record of structured clinical interview ( VSI ) assessed by an independent rater out of five psychiatrists .
	manualset3
195100	3	415889	7	NULL	NULL	0	NULL	depressive symptomatology improvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two different methods were compared in the assessment of depressive symptomatology improvement : live naturalistic ( N ) performed by the patient 's therapist , and from videotape record of structured clinical interview ( VSI ) assessed by an independent rater out of five psychiatrists .
	manualset3
195101	4	415889	7	NULL	NULL	0	NULL	 live naturalistic ( N )	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two different methods were compared in the assessment of depressive symptomatology improvement : live naturalistic ( N ) performed by the patient 's therapist , and from videotape record of structured clinical interview ( VSI ) assessed by an independent rater out of five psychiatrists .
	manualset3
195102	5	415889	7	NULL	NULL	0	NULL	patient 's therapist	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two different methods were compared in the assessment of depressive symptomatology improvement : live naturalistic ( N ) performed by the patient 's therapist , and from videotape record of structured clinical interview ( VSI ) assessed by an independent rater out of five psychiatrists .
	manualset3
195103	6	415889	7	NULL	NULL	0	NULL	videotape record 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two different methods were compared in the assessment of depressive symptomatology improvement : live naturalistic ( N ) performed by the patient 's therapist , and from videotape record of structured clinical interview ( VSI ) assessed by an independent rater out of five psychiatrists .
	manualset3
195104	7	415889	7	NULL	NULL	0	NULL	structured clinical interview ( VSI ) 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Two different methods were compared in the assessment of depressive symptomatology improvement : live naturalistic ( N ) performed by the patient 's therapist , and from videotape record of structured clinical interview ( VSI ) assessed by an independent rater out of five psychiatrists .
	manualset3
195105	8	415889	7	NULL	NULL	0	NULL	independent rater	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Two different methods were compared in the assessment of depressive symptomatology improvement : live naturalistic ( N ) performed by the patient 's therapist , and from videotape record of structured clinical interview ( VSI ) assessed by an independent rater out of five psychiatrists .
	manualset3
195106	9	415889	7	NULL	NULL	0	NULL	 five psychiatrists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two different methods were compared in the assessment of depressive symptomatology improvement : live naturalistic ( N ) performed by the patient 's therapist , and from videotape record of structured clinical interview ( VSI ) assessed by an independent rater out of five psychiatrists .
	manualset3
195107	1	415890	7	NULL	NULL	0	NULL	Two different subsets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Two different subsets of T cells , Th1 and Th2 cells , have been demonstrated to secrete different profiles of cytokines and to influence various infections in different ways .
	manualset3
195109	2	415890	7	NULL	NULL	0	NULL	T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Two different subsets of T cells , Th1 and Th2 cells , have been demonstrated to secrete different profiles of cytokines and to influence various infections in different ways .
	manualset3
195110	3	415890	7	NULL	NULL	0	NULL	 Th1 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Two different subsets of T cells , Th1 and Th2 cells , have been demonstrated to secrete different profiles of cytokines and to influence various infections in different ways .
	manualset3
195111	4	415890	7	NULL	NULL	0	NULL	Th2 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Two different subsets of T cells , Th1 and Th2 cells , have been demonstrated to secrete different profiles of cytokines and to influence various infections in different ways .
	manualset3
195113	5	415890	7	NULL	NULL	NULL	NULL	different profiles	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two different subsets of T cells , Th1 and Th2 cells , have been demonstrated to secrete different profiles of cytokines and to influence various infections in different ways .
	manualset3
195114	6	415890	7	NULL	NULL	0	NULL	cytokines	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Two different subsets of T cells , Th1 and Th2 cells , have been demonstrated to secrete different profiles of cytokines and to influence various infections in different ways .
	manualset3
195116	7	415890	7	NULL	NULL	0	NULL	infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two different subsets of T cells , Th1 and Th2 cells , have been demonstrated to secrete different profiles of cytokines and to influence various infections in different ways .
	manualset3
195118	8	415890	7	NULL	NULL	0	NULL	different ways	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two different subsets of T cells , Th1 and Th2 cells , have been demonstrated to secrete different profiles of cytokines and to influence various infections in different ways .
	manualset3
195120	1	415891	7	NULL	NULL	NULL	NULL	Two different types of stimuli	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two different types of stimuli were used : flash and checkerboard pattern .
	manualset3
195123	3	415891	7	NULL	NULL	0	NULL	flash and checkerboard pattern	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two different types of stimuli were used : flash and checkerboard pattern .
	manualset3
195126	1	415892	7	NULL	NULL	0	NULL	Two distinct areas	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two distinct areas of endemic chromoblastomycosis , each with a characteristic ecosystem and a single species , are identified .
	manualset3
195127	2	415892	7	NULL	NULL	0	NULL	endemic chromoblastomycosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two distinct areas of endemic chromoblastomycosis , each with a characteristic ecosystem and a single species , are identified .
	manualset3
195128	3	415892	7	NULL	NULL	0	NULL	ecosystem 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Two distinct areas of endemic chromoblastomycosis , each with a characteristic ecosystem and a single species , are identified .
	manualset3
195129	4	415892	7	NULL	NULL	0	NULL	 single species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two distinct areas of endemic chromoblastomycosis , each with a characteristic ecosystem and a single species , are identified .
	manualset3
195132	1	415893	7	NULL	NULL	0	NULL	 IFs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After removing IFs by calcination , electron microscopy revealed hollow silica nanotubes several micrometers long , with outer diameters of 35-55 nm and an average inner diameter of 10 nm ( comparable to that of IFs ) .
	manualset3
195133	2	415893	7	NULL	NULL	0	NULL	calcination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After removing IFs by calcination , electron microscopy revealed hollow silica nanotubes several micrometers long , with outer diameters of 35-55 nm and an average inner diameter of 10 nm ( comparable to that of IFs ) .
	manualset3
195134	3	415893	7	NULL	NULL	0	NULL	electron microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After removing IFs by calcination , electron microscopy revealed hollow silica nanotubes several micrometers long , with outer diameters of 35-55 nm and an average inner diameter of 10 nm ( comparable to that of IFs ) .
	manualset3
195135	4	415893	7	NULL	NULL	0	NULL	hollow silica nanotubes	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	After removing IFs by calcination , electron microscopy revealed hollow silica nanotubes several micrometers long , with outer diameters of 35-55 nm and an average inner diameter of 10 nm ( comparable to that of IFs ) .
	manualset3
195136	5	415893	7	NULL	NULL	0	NULL	micrometers long	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After removing IFs by calcination , electron microscopy revealed hollow silica nanotubes several micrometers long , with outer diameters of 35-55 nm and an average inner diameter of 10 nm ( comparable to that of IFs ) .
	manualset3
195137	6	415893	7	NULL	NULL	0	NULL	outer diameters	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After removing IFs by calcination , electron microscopy revealed hollow silica nanotubes several micrometers long , with outer diameters of 35-55 nm and an average inner diameter of 10 nm ( comparable to that of IFs ) .
	manualset3
195138	7	415893	7	NULL	NULL	0	NULL	35-55 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	After removing IFs by calcination , electron microscopy revealed hollow silica nanotubes several micrometers long , with outer diameters of 35-55 nm and an average inner diameter of 10 nm ( comparable to that of IFs ) .
	manualset3
195139	8	415893	7	NULL	NULL	0	NULL	average inner diameter	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After removing IFs by calcination , electron microscopy revealed hollow silica nanotubes several micrometers long , with outer diameters of 35-55 nm and an average inner diameter of 10 nm ( comparable to that of IFs ) .
	manualset3
195140	9	415893	7	NULL	NULL	0	NULL	10 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	After removing IFs by calcination , electron microscopy revealed hollow silica nanotubes several micrometers long , with outer diameters of 35-55 nm and an average inner diameter of 10 nm ( comparable to that of IFs ) .
	manualset3
195141	10	415893	7	NULL	NULL	0	NULL	IFs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After removing IFs by calcination , electron microscopy revealed hollow silica nanotubes several micrometers long , with outer diameters of 35-55 nm and an average inner diameter of 10 nm ( comparable to that of IFs ) .
	manualset3
195142	1	415894	7	NULL	NULL	0	NULL	Two distinct human POM121 genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two distinct human POM121 genes : requirement for the formation of nuclear pore complexes .
	manualset3
195143	2	415894	7	NULL	NULL	0	NULL	formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two distinct human POM121 genes : requirement for the formation of nuclear pore complexes .
	manualset3
195144	3	415894	7	NULL	NULL	0	NULL	nuclear pore complexes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Two distinct human POM121 genes : requirement for the formation of nuclear pore complexes .
	manualset3
195145	4	415894	7	NULL	NULL	0	NULL	requirement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two distinct human POM121 genes : requirement for the formation of nuclear pore complexes .
	manualset3
195146	1	415895	7	NULL	NULL	0	NULL	Two distinct subtypes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two distinct subtypes of hepatitis B virus-related acute liver failure are separable by quantitative serum immunoglobulin M anti-hepatitis B core antibody and hepatitis B virus DNA levels .
	manualset3
195147	2	415895	7	NULL	NULL	0	NULL	hepatitis B virus-related acute liver failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two distinct subtypes of hepatitis B virus-related acute liver failure are separable by quantitative serum immunoglobulin M anti-hepatitis B core antibody and hepatitis B virus DNA levels .
	manualset3
195148	3	415895	7	NULL	NULL	0	NULL	quantitative serum immunoglobulin M anti-hepatitis B core antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Two distinct subtypes of hepatitis B virus-related acute liver failure are separable by quantitative serum immunoglobulin M anti-hepatitis B core antibody and hepatitis B virus DNA levels .
	manualset3
195149	4	415895	7	NULL	NULL	0	NULL	hepatitis B virus DNA levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two distinct subtypes of hepatitis B virus-related acute liver failure are separable by quantitative serum immunoglobulin M anti-hepatitis B core antibody and hepatitis B virus DNA levels .
	manualset3
195150	1	415896	7	NULL	NULL	0	NULL	Two disulfide-linked surface proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two disulfide-linked surface proteins expressed by LH8-105 cells have been positively identified by immunoprecipitation with specific antisera .
	manualset3
195151	2	415896	7	NULL	NULL	0	NULL	LH8-105 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Two disulfide-linked surface proteins expressed by LH8-105 cells have been positively identified by immunoprecipitation with specific antisera .
	manualset3
195152	3	415896	7	NULL	NULL	0	NULL	immunoprecipitation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two disulfide-linked surface proteins expressed by LH8-105 cells have been positively identified by immunoprecipitation with specific antisera .
	manualset3
195153	4	415896	7	NULL	NULL	0	NULL	specific antisera	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two disulfide-linked surface proteins expressed by LH8-105 cells have been positively identified by immunoprecipitation with specific antisera .
	manualset3
195191	1	415897	7	NULL	NULL	0	NULL	Two evolutionally unrelated Thy enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two evolutionally unrelated Thy enzymes , ThyA and ThyX , are known to catalyze the same biochemical reaction .
	manualset3
195192	2	415897	7	NULL	NULL	0	NULL	ThyA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Two evolutionally unrelated Thy enzymes , ThyA and ThyX , are known to catalyze the same biochemical reaction .
	manualset3
195193	3	415897	7	NULL	NULL	0	NULL	ThyX	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Two evolutionally unrelated Thy enzymes , ThyA and ThyX , are known to catalyze the same biochemical reaction .
	manualset3
195194	4	415897	7	NULL	NULL	0	NULL	biochemical reaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two evolutionally unrelated Thy enzymes , ThyA and ThyX , are known to catalyze the same biochemical reaction .
	manualset3
195195	1	415898	7	NULL	NULL	0	NULL	Two experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were conducted to examine the hypothesis that learning by analogy will invoke characteristics of an implicit mode of motor learning .
	manualset3
195196	2	415898	7	NULL	NULL	0	NULL	 hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were conducted to examine the hypothesis that learning by analogy will invoke characteristics of an implicit mode of motor learning .
	manualset3
195197	3	415898	7	NULL	NULL	0	NULL	learning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were conducted to examine the hypothesis that learning by analogy will invoke characteristics of an implicit mode of motor learning .
	manualset3
195198	4	415898	7	NULL	NULL	0	NULL	analogy	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were conducted to examine the hypothesis that learning by analogy will invoke characteristics of an implicit mode of motor learning .
	manualset3
195199	5	415898	7	NULL	NULL	0	NULL	 implicit mode	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were conducted to examine the hypothesis that learning by analogy will invoke characteristics of an implicit mode of motor learning .
	manualset3
195200	6	415898	7	NULL	NULL	0	NULL	motor learning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were conducted to examine the hypothesis that learning by analogy will invoke characteristics of an implicit mode of motor learning .
	manualset3
195201	1	415899	7	NULL	NULL	0	NULL	Two experiments 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were conducted to examine whether the conclusions drawn regarding the timing of anticipatory information pick-up from temporal occlusion studies are influenced by whether ( a ) the viewing period is of variable or fixed duration and ( b ) the task is a laboratory-based one with simple responses or a natural one requiring a coupled , interceptive movement response .
	manualset3
195202	2	415899	7	NULL	NULL	0	NULL	conclusions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were conducted to examine whether the conclusions drawn regarding the timing of anticipatory information pick-up from temporal occlusion studies are influenced by whether ( a ) the viewing period is of variable or fixed duration and ( b ) the task is a laboratory-based one with simple responses or a natural one requiring a coupled , interceptive movement response .
	manualset3
195203	3	415899	7	NULL	NULL	0	NULL	 timing 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were conducted to examine whether the conclusions drawn regarding the timing of anticipatory information pick-up from temporal occlusion studies are influenced by whether ( a ) the viewing period is of variable or fixed duration and ( b ) the task is a laboratory-based one with simple responses or a natural one requiring a coupled , interceptive movement response .
	manualset3
195204	4	415899	7	NULL	NULL	0	NULL	anticipatory information pick-up	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were conducted to examine whether the conclusions drawn regarding the timing of anticipatory information pick-up from temporal occlusion studies are influenced by whether ( a ) the viewing period is of variable or fixed duration and ( b ) the task is a laboratory-based one with simple responses or a natural one requiring a coupled , interceptive movement response .
	manualset3
195205	5	415899	7	NULL	NULL	0	NULL	temporal occlusion studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were conducted to examine whether the conclusions drawn regarding the timing of anticipatory information pick-up from temporal occlusion studies are influenced by whether ( a ) the viewing period is of variable or fixed duration and ( b ) the task is a laboratory-based one with simple responses or a natural one requiring a coupled , interceptive movement response .
	manualset3
195206	6	415899	7	NULL	NULL	0	NULL	 viewing period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were conducted to examine whether the conclusions drawn regarding the timing of anticipatory information pick-up from temporal occlusion studies are influenced by whether ( a ) the viewing period is of variable or fixed duration and ( b ) the task is a laboratory-based one with simple responses or a natural one requiring a coupled , interceptive movement response .
	manualset3
195207	7	415899	7	NULL	NULL	0	NULL	variable duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were conducted to examine whether the conclusions drawn regarding the timing of anticipatory information pick-up from temporal occlusion studies are influenced by whether ( a ) the viewing period is of variable or fixed duration and ( b ) the task is a laboratory-based one with simple responses or a natural one requiring a coupled , interceptive movement response .
	manualset3
195208	8	415899	7	NULL	NULL	0	NULL	fixed duration 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were conducted to examine whether the conclusions drawn regarding the timing of anticipatory information pick-up from temporal occlusion studies are influenced by whether ( a ) the viewing period is of variable or fixed duration and ( b ) the task is a laboratory-based one with simple responses or a natural one requiring a coupled , interceptive movement response .
	manualset3
195209	9	415899	7	NULL	NULL	0	NULL	 task	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were conducted to examine whether the conclusions drawn regarding the timing of anticipatory information pick-up from temporal occlusion studies are influenced by whether ( a ) the viewing period is of variable or fixed duration and ( b ) the task is a laboratory-based one with simple responses or a natural one requiring a coupled , interceptive movement response .
	manualset3
195210	10	415899	7	NULL	NULL	0	NULL	laboratory-based one	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were conducted to examine whether the conclusions drawn regarding the timing of anticipatory information pick-up from temporal occlusion studies are influenced by whether ( a ) the viewing period is of variable or fixed duration and ( b ) the task is a laboratory-based one with simple responses or a natural one requiring a coupled , interceptive movement response .
	manualset3
195211	11	415899	7	NULL	NULL	0	NULL	simple responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were conducted to examine whether the conclusions drawn regarding the timing of anticipatory information pick-up from temporal occlusion studies are influenced by whether ( a ) the viewing period is of variable or fixed duration and ( b ) the task is a laboratory-based one with simple responses or a natural one requiring a coupled , interceptive movement response .
	manualset3
195212	12	415899	7	NULL	NULL	0	NULL	natural one	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were conducted to examine whether the conclusions drawn regarding the timing of anticipatory information pick-up from temporal occlusion studies are influenced by whether ( a ) the viewing period is of variable or fixed duration and ( b ) the task is a laboratory-based one with simple responses or a natural one requiring a coupled , interceptive movement response .
	manualset3
195213	13	415899	7	NULL	NULL	0	NULL	coupled , interceptive movement response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were conducted to examine whether the conclusions drawn regarding the timing of anticipatory information pick-up from temporal occlusion studies are influenced by whether ( a ) the viewing period is of variable or fixed duration and ( b ) the task is a laboratory-based one with simple responses or a natural one requiring a coupled , interceptive movement response .
	manualset3
195214	1	415900	7	NULL	NULL	0	NULL	Two experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were performed to determine the effect of low EST at the start of incubation and high EST at the end of incubation on hatchability , chick quality , 6-wk live performance , and breast meat yield of broiler chickens .
	manualset3
195215	2	415900	7	NULL	NULL	0	NULL	 effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were performed to determine the effect of low EST at the start of incubation and high EST at the end of incubation on hatchability , chick quality , 6-wk live performance , and breast meat yield of broiler chickens .
	manualset3
195216	3	415900	7	NULL	NULL	0	NULL	 low EST	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were performed to determine the effect of low EST at the start of incubation and high EST at the end of incubation on hatchability , chick quality , 6-wk live performance , and breast meat yield of broiler chickens .
	manualset3
195217	4	415900	7	NULL	NULL	0	NULL	start	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were performed to determine the effect of low EST at the start of incubation and high EST at the end of incubation on hatchability , chick quality , 6-wk live performance , and breast meat yield of broiler chickens .
	manualset3
195218	5	415900	7	NULL	NULL	0	NULL	incubation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were performed to determine the effect of low EST at the start of incubation and high EST at the end of incubation on hatchability , chick quality , 6-wk live performance , and breast meat yield of broiler chickens .
	manualset3
195219	6	415900	7	NULL	NULL	0	NULL	high EST	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were performed to determine the effect of low EST at the start of incubation and high EST at the end of incubation on hatchability , chick quality , 6-wk live performance , and breast meat yield of broiler chickens .
	manualset3
195220	7	415900	7	NULL	NULL	0	NULL	 end	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were performed to determine the effect of low EST at the start of incubation and high EST at the end of incubation on hatchability , chick quality , 6-wk live performance , and breast meat yield of broiler chickens .
	manualset3
195221	8	415900	7	NULL	NULL	0	NULL	 incubation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were performed to determine the effect of low EST at the start of incubation and high EST at the end of incubation on hatchability , chick quality , 6-wk live performance , and breast meat yield of broiler chickens .
	manualset3
195222	9	415900	7	NULL	NULL	0	NULL	hatchability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were performed to determine the effect of low EST at the start of incubation and high EST at the end of incubation on hatchability , chick quality , 6-wk live performance , and breast meat yield of broiler chickens .
	manualset3
195223	10	415900	7	NULL	NULL	0	NULL	chick quality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were performed to determine the effect of low EST at the start of incubation and high EST at the end of incubation on hatchability , chick quality , 6-wk live performance , and breast meat yield of broiler chickens .
	manualset3
195224	11	415900	7	NULL	NULL	0	NULL	6-wk live performance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were performed to determine the effect of low EST at the start of incubation and high EST at the end of incubation on hatchability , chick quality , 6-wk live performance , and breast meat yield of broiler chickens .
	manualset3
195225	12	415900	7	NULL	NULL	0	NULL	breast meat yield	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were performed to determine the effect of low EST at the start of incubation and high EST at the end of incubation on hatchability , chick quality , 6-wk live performance , and breast meat yield of broiler chickens .
	manualset3
195226	13	415900	7	NULL	NULL	0	NULL	broiler chickens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two experiments were performed to determine the effect of low EST at the start of incubation and high EST at the end of incubation on hatchability , chick quality , 6-wk live performance , and breast meat yield of broiler chickens .
	manualset3
195227	1	415901	7	NULL	NULL	0	NULL	Two factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two factors could influence the result significantly , i.e. , source of animal and number of sham exposures .
	manualset3
195228	2	415901	7	NULL	NULL	0	NULL	result	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two factors could influence the result significantly , i.e. , source of animal and number of sham exposures .
	manualset3
195229	3	415901	7	NULL	NULL	NULL	NULL	source of animal	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two factors could influence the result significantly , i.e. , source of animal and number of sham exposures .
	manualset3
195230	4	415901	7	NULL	NULL	0	NULL	 number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two factors could influence the result significantly , i.e. , source of animal and number of sham exposures .
	manualset3
195231	5	415901	7	NULL	NULL	0	NULL	sham exposures 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two factors could influence the result significantly , i.e. , source of animal and number of sham exposures .
	manualset3
195232	1	415902	7	NULL	NULL	0	NULL	Two field isolates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two field isolates of Eimeria tenella were isolated on farms where continuous outbreaks of coccidiosis in broilers had occurred over several years .
	manualset3
195233	2	415902	7	NULL	NULL	0	NULL	Eimeria tenella	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two field isolates of Eimeria tenella were isolated on farms where continuous outbreaks of coccidiosis in broilers had occurred over several years .
	manualset3
195234	3	415902	7	NULL	NULL	0	NULL	farms	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Two field isolates of Eimeria tenella were isolated on farms where continuous outbreaks of coccidiosis in broilers had occurred over several years .
	manualset3
195235	4	415902	7	NULL	NULL	0	NULL	continuous outbreaks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two field isolates of Eimeria tenella were isolated on farms where continuous outbreaks of coccidiosis in broilers had occurred over several years .
	manualset3
195236	5	415902	7	NULL	NULL	0	NULL	coccidiosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two field isolates of Eimeria tenella were isolated on farms where continuous outbreaks of coccidiosis in broilers had occurred over several years .
	manualset3
195237	6	415902	7	NULL	NULL	0	NULL	broilers	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two field isolates of Eimeria tenella were isolated on farms where continuous outbreaks of coccidiosis in broilers had occurred over several years .
	manualset3
195238	7	415902	7	NULL	NULL	0	NULL	several years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Two field isolates of Eimeria tenella were isolated on farms where continuous outbreaks of coccidiosis in broilers had occurred over several years .
	manualset3
195239	1	415903	7	NULL	NULL	0	NULL	Congenital aneurysmal dilatation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Congenital aneurysmal dilatation of left atrium ( author 's transl ) ) .
	manualset3
195240	2	415903	7	NULL	NULL	0	NULL	left atrium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Congenital aneurysmal dilatation of left atrium ( author 's transl ) ) .
	manualset3
195241	3	415903	7	NULL	NULL	0	NULL	author 's transl	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Congenital aneurysmal dilatation of left atrium ( author 's transl ) ) .
	manualset3
195300	1	415904	7	NULL	NULL	0	NULL	Two formulas	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Two formulas of nearly identical composition except for iron concentration ( 10.2 and 2.5 mg/L ) were fed .
	manualset3
195301	2	415904	7	NULL	NULL	0	NULL	identical composition	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two formulas of nearly identical composition except for iron concentration ( 10.2 and 2.5 mg/L ) were fed .
	manualset3
195302	3	415904	7	NULL	NULL	0	NULL	iron concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two formulas of nearly identical composition except for iron concentration ( 10.2 and 2.5 mg/L ) were fed .
	manualset3
195303	4	415904	7	NULL	NULL	0	NULL	10.2 mg/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Two formulas of nearly identical composition except for iron concentration ( 10.2 and 2.5 mg/L ) were fed .
	manualset3
195304	5	415904	7	NULL	NULL	0	NULL	2.5 mg/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Two formulas of nearly identical composition except for iron concentration ( 10.2 and 2.5 mg/L ) were fed .
	manualset3
195305	1	415905	7	NULL	NULL	0	NULL	Two human lymphoblastoid cell lineages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Two human lymphoblastoid cell lineages derived from the same parental line exhibit markedly different survival and mutational responses to X-irradiation , but not to chemical point mutagens .
	manualset3
195306	2	415905	7	NULL	NULL	0	NULL	same parental line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Two human lymphoblastoid cell lineages derived from the same parental line exhibit markedly different survival and mutational responses to X-irradiation , but not to chemical point mutagens .
	manualset3
195307	3	415905	7	NULL	NULL	0	NULL	 different survival 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two human lymphoblastoid cell lineages derived from the same parental line exhibit markedly different survival and mutational responses to X-irradiation , but not to chemical point mutagens .
	manualset3
195308	4	415905	7	NULL	NULL	0	NULL	 mutational responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two human lymphoblastoid cell lineages derived from the same parental line exhibit markedly different survival and mutational responses to X-irradiation , but not to chemical point mutagens .
	manualset3
195309	5	415905	7	NULL	NULL	0	NULL	X-irradiation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Two human lymphoblastoid cell lineages derived from the same parental line exhibit markedly different survival and mutational responses to X-irradiation , but not to chemical point mutagens .
	manualset3
195310	6	415905	7	NULL	NULL	0	NULL	chemical point mutagens 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two human lymphoblastoid cell lineages derived from the same parental line exhibit markedly different survival and mutational responses to X-irradiation , but not to chemical point mutagens .
	manualset3
195311	1	415906	7	NULL	NULL	0	NULL	Two hydrogen-bonds	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two hydrogen-bonds from geometrically constrained OH groups to coordinated oxygen donors shift the reduction potential of a Cu ( II ) complex by +270 mV as compared to the structurally analogous reference complex missing the OH groups .
	manualset3
195312	2	415906	7	NULL	NULL	0	NULL	geometrically constrained OH groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two hydrogen-bonds from geometrically constrained OH groups to coordinated oxygen donors shift the reduction potential of a Cu ( II ) complex by +270 mV as compared to the structurally analogous reference complex missing the OH groups .
	manualset3
195313	3	415906	7	NULL	NULL	0	NULL	coordinated oxygen donors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two hydrogen-bonds from geometrically constrained OH groups to coordinated oxygen donors shift the reduction potential of a Cu ( II ) complex by +270 mV as compared to the structurally analogous reference complex missing the OH groups .
	manualset3
195314	4	415906	7	NULL	NULL	0	NULL	reduction potential	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two hydrogen-bonds from geometrically constrained OH groups to coordinated oxygen donors shift the reduction potential of a Cu ( II ) complex by +270 mV as compared to the structurally analogous reference complex missing the OH groups .
	manualset3
195315	5	415906	7	NULL	NULL	0	NULL	Cu ( II ) complex	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two hydrogen-bonds from geometrically constrained OH groups to coordinated oxygen donors shift the reduction potential of a Cu ( II ) complex by +270 mV as compared to the structurally analogous reference complex missing the OH groups .
	manualset3
195316	6	415906	7	NULL	NULL	0	NULL	+270 mV	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Two hydrogen-bonds from geometrically constrained OH groups to coordinated oxygen donors shift the reduction potential of a Cu ( II ) complex by +270 mV as compared to the structurally analogous reference complex missing the OH groups .
	manualset3
195317	7	415906	7	NULL	NULL	0	NULL	structurally analogous reference complex 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two hydrogen-bonds from geometrically constrained OH groups to coordinated oxygen donors shift the reduction potential of a Cu ( II ) complex by +270 mV as compared to the structurally analogous reference complex missing the OH groups .
	manualset3
195318	8	415906	7	NULL	NULL	0	NULL	OH groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two hydrogen-bonds from geometrically constrained OH groups to coordinated oxygen donors shift the reduction potential of a Cu ( II ) complex by +270 mV as compared to the structurally analogous reference complex missing the OH groups .
	manualset3
195319	1	415907	7	NULL	NULL	0	NULL	Two independent programs	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Two independent programs appear to operate , one that is blocked by ABA , governing developmental growth resulting in germination ; and a second that governs storage lipid mobilization which is largely ABA-independent .
	manualset3
195320	2	415907	7	NULL	NULL	0	NULL	 one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two independent programs appear to operate , one that is blocked by ABA , governing developmental growth resulting in germination ; and a second that governs storage lipid mobilization which is largely ABA-independent .
	manualset3
195321	3	415907	7	NULL	NULL	0	NULL	ABA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two independent programs appear to operate , one that is blocked by ABA , governing developmental growth resulting in germination ; and a second that governs storage lipid mobilization which is largely ABA-independent .
	manualset3
195322	4	415907	7	NULL	NULL	0	NULL	developmental growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two independent programs appear to operate , one that is blocked by ABA , governing developmental growth resulting in germination ; and a second that governs storage lipid mobilization which is largely ABA-independent .
	manualset3
195323	5	415907	7	NULL	NULL	0	NULL	germination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two independent programs appear to operate , one that is blocked by ABA , governing developmental growth resulting in germination ; and a second that governs storage lipid mobilization which is largely ABA-independent .
	manualset3
195324	6	415907	7	NULL	NULL	0	NULL	second 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two independent programs appear to operate , one that is blocked by ABA , governing developmental growth resulting in germination ; and a second that governs storage lipid mobilization which is largely ABA-independent .
	manualset3
195325	7	415907	7	NULL	NULL	0	NULL	lipid mobilization 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two independent programs appear to operate , one that is blocked by ABA , governing developmental growth resulting in germination ; and a second that governs storage lipid mobilization which is largely ABA-independent .
	manualset3
195326	8	415907	7	NULL	NULL	0	NULL	ABA-independent 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two independent programs appear to operate , one that is blocked by ABA , governing developmental growth resulting in germination ; and a second that governs storage lipid mobilization which is largely ABA-independent .
	manualset3
195327	1	415908	7	NULL	NULL	0	NULL	Two infusion paradigms	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Two infusion paradigms were studied , each with 1.5-mg / kg hourly dose for 4 hours -- steady infusion and pulse infusion of the full hour dose over 5 minutes each hour .
	manualset3
195328	2	415908	7	NULL	NULL	0	NULL	1.5-mg / kg hourly dose 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two infusion paradigms were studied , each with 1.5-mg / kg hourly dose for 4 hours -- steady infusion and pulse infusion of the full hour dose over 5 minutes each hour .
	manualset3
195329	3	415908	7	NULL	NULL	0	NULL	4 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Two infusion paradigms were studied , each with 1.5-mg / kg hourly dose for 4 hours -- steady infusion and pulse infusion of the full hour dose over 5 minutes each hour .
	manualset3
195330	4	415908	7	NULL	NULL	0	NULL	steady infusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two infusion paradigms were studied , each with 1.5-mg / kg hourly dose for 4 hours -- steady infusion and pulse infusion of the full hour dose over 5 minutes each hour .
	manualset3
195331	5	415908	7	NULL	NULL	0	NULL	pulse infusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two infusion paradigms were studied , each with 1.5-mg / kg hourly dose for 4 hours -- steady infusion and pulse infusion of the full hour dose over 5 minutes each hour .
	manualset3
195332	6	415908	7	NULL	NULL	0	NULL	full hour dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two infusion paradigms were studied , each with 1.5-mg / kg hourly dose for 4 hours -- steady infusion and pulse infusion of the full hour dose over 5 minutes each hour .
	manualset3
195333	7	415908	7	NULL	NULL	0	NULL	 5 minutes	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Two infusion paradigms were studied , each with 1.5-mg / kg hourly dose for 4 hours -- steady infusion and pulse infusion of the full hour dose over 5 minutes each hour .
	manualset3
195334	8	415908	7	NULL	NULL	0	NULL	hour	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Two infusion paradigms were studied , each with 1.5-mg / kg hourly dose for 4 hours -- steady infusion and pulse infusion of the full hour dose over 5 minutes each hour .
	manualset3
195335	1	415909	7	NULL	NULL	0	NULL	Two isoforms ,	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two isoforms , Gat1p/Gpt2p and Gat2p/Sct1p , are present in the yeast Saccharomyces cerevisiae .
	manualset3
195336	2	415909	7	NULL	NULL	0	NULL	Gat1p/Gpt2p	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Two isoforms , Gat1p/Gpt2p and Gat2p/Sct1p , are present in the yeast Saccharomyces cerevisiae .
	manualset3
195337	3	415909	7	NULL	NULL	0	NULL	Gat2p/Sct1p	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Two isoforms , Gat1p/Gpt2p and Gat2p/Sct1p , are present in the yeast Saccharomyces cerevisiae .
	manualset3
195338	4	415909	7	NULL	NULL	0	NULL	yeast Saccharomyces cerevisiae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two isoforms , Gat1p/Gpt2p and Gat2p/Sct1p , are present in the yeast Saccharomyces cerevisiae .
	manualset3
195363	1	415910	7	NULL	NULL	0	NULL	resolution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After resolution of discrepant test results by use of additional PCR assays targeting other viral genes , the sensitivity ( Se ) and specificity ( Sp ) of the multiplex PCR assay for influenza A virus were 100 and 97.7 % compared to 43.6 and 98.5 % for the antigenic test .
	manualset3
195364	2	415910	7	NULL	NULL	0	NULL	discrepant test results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After resolution of discrepant test results by use of additional PCR assays targeting other viral genes , the sensitivity ( Se ) and specificity ( Sp ) of the multiplex PCR assay for influenza A virus were 100 and 97.7 % compared to 43.6 and 98.5 % for the antigenic test .
	manualset3
195365	3	415910	7	NULL	NULL	0	NULL	PCR assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After resolution of discrepant test results by use of additional PCR assays targeting other viral genes , the sensitivity ( Se ) and specificity ( Sp ) of the multiplex PCR assay for influenza A virus were 100 and 97.7 % compared to 43.6 and 98.5 % for the antigenic test .
	manualset3
195366	4	415910	7	NULL	NULL	0	NULL	 viral genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	After resolution of discrepant test results by use of additional PCR assays targeting other viral genes , the sensitivity ( Se ) and specificity ( Sp ) of the multiplex PCR assay for influenza A virus were 100 and 97.7 % compared to 43.6 and 98.5 % for the antigenic test .
	manualset3
195367	5	415910	7	NULL	NULL	0	NULL	 sensitivity ( Se )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After resolution of discrepant test results by use of additional PCR assays targeting other viral genes , the sensitivity ( Se ) and specificity ( Sp ) of the multiplex PCR assay for influenza A virus were 100 and 97.7 % compared to 43.6 and 98.5 % for the antigenic test .
	manualset3
195368	6	415910	7	NULL	NULL	0	NULL	specificity ( Sp ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After resolution of discrepant test results by use of additional PCR assays targeting other viral genes , the sensitivity ( Se ) and specificity ( Sp ) of the multiplex PCR assay for influenza A virus were 100 and 97.7 % compared to 43.6 and 98.5 % for the antigenic test .
	manualset3
195369	7	415910	7	NULL	NULL	0	NULL	multiplex PCR assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After resolution of discrepant test results by use of additional PCR assays targeting other viral genes , the sensitivity ( Se ) and specificity ( Sp ) of the multiplex PCR assay for influenza A virus were 100 and 97.7 % compared to 43.6 and 98.5 % for the antigenic test .
	manualset3
195370	8	415910	7	NULL	NULL	0	NULL	influenza A virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	After resolution of discrepant test results by use of additional PCR assays targeting other viral genes , the sensitivity ( Se ) and specificity ( Sp ) of the multiplex PCR assay for influenza A virus were 100 and 97.7 % compared to 43.6 and 98.5 % for the antigenic test .
	manualset3
195371	9	415910	7	NULL	NULL	0	NULL	100%	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After resolution of discrepant test results by use of additional PCR assays targeting other viral genes , the sensitivity ( Se ) and specificity ( Sp ) of the multiplex PCR assay for influenza A virus were 100 and 97.7 % compared to 43.6 and 98.5 % for the antigenic test .
	manualset3
195372	10	415910	7	NULL	NULL	0	NULL	97.7 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After resolution of discrepant test results by use of additional PCR assays targeting other viral genes , the sensitivity ( Se ) and specificity ( Sp ) of the multiplex PCR assay for influenza A virus were 100 and 97.7 % compared to 43.6 and 98.5 % for the antigenic test .
	manualset3
195373	11	415910	7	NULL	NULL	0	NULL	43.6%	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After resolution of discrepant test results by use of additional PCR assays targeting other viral genes , the sensitivity ( Se ) and specificity ( Sp ) of the multiplex PCR assay for influenza A virus were 100 and 97.7 % compared to 43.6 and 98.5 % for the antigenic test .
	manualset3
195374	12	415910	7	NULL	NULL	0	NULL	98.5 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After resolution of discrepant test results by use of additional PCR assays targeting other viral genes , the sensitivity ( Se ) and specificity ( Sp ) of the multiplex PCR assay for influenza A virus were 100 and 97.7 % compared to 43.6 and 98.5 % for the antigenic test .
	manualset3
195375	13	415910	7	NULL	NULL	0	NULL	antigenic test 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After resolution of discrepant test results by use of additional PCR assays targeting other viral genes , the sensitivity ( Se ) and specificity ( Sp ) of the multiplex PCR assay for influenza A virus were 100 and 97.7 % compared to 43.6 and 98.5 % for the antigenic test .
	manualset3
195376	1	415911	7	NULL	NULL	0	NULL	Two major approaches	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two major approaches provided encouraging results when used in spontaneous models of autoimmune diabetes that are the use of - cell autoantigens and of monoclonal antibodies to CD3 .
	manualset3
195377	2	415911	7	NULL	NULL	0	NULL	encouraging results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two major approaches provided encouraging results when used in spontaneous models of autoimmune diabetes that are the use of - cell autoantigens and of monoclonal antibodies to CD3 .
	manualset3
195378	3	415911	7	NULL	NULL	NULL	NULL	spontaneous models	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two major approaches provided encouraging results when used in spontaneous models of autoimmune diabetes that are the use of - cell autoantigens and of monoclonal antibodies to CD3 .
	manualset3
195379	4	415911	7	NULL	NULL	0	NULL	autoimmune diabetes 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two major approaches provided encouraging results when used in spontaneous models of autoimmune diabetes that are the use of - cell autoantigens and of monoclonal antibodies to CD3 .
	manualset3
195380	5	415911	7	NULL	NULL	0	NULL	cell autoantigens	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two major approaches provided encouraging results when used in spontaneous models of autoimmune diabetes that are the use of - cell autoantigens and of monoclonal antibodies to CD3 .
	manualset3
195381	6	415911	7	NULL	NULL	0	NULL	monoclonal antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two major approaches provided encouraging results when used in spontaneous models of autoimmune diabetes that are the use of - cell autoantigens and of monoclonal antibodies to CD3 .
	manualset3
195382	7	415911	7	NULL	NULL	0	NULL	CD3	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Two major approaches provided encouraging results when used in spontaneous models of autoimmune diabetes that are the use of - cell autoantigens and of monoclonal antibodies to CD3 .
	manualset3
195383	1	415912	7	NULL	NULL	0	NULL	Two milliliters	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two milliliters of samples containing N-propylprocainamide as the internal standard are buffered to pH 9 and extracted with n-butyl chloride .
	manualset3
195384	2	415912	7	NULL	NULL	0	NULL	samples	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two milliliters of samples containing N-propylprocainamide as the internal standard are buffered to pH 9 and extracted with n-butyl chloride .
	manualset3
195385	3	415912	7	NULL	NULL	0	NULL	N-propylprocainamide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two milliliters of samples containing N-propylprocainamide as the internal standard are buffered to pH 9 and extracted with n-butyl chloride .
	manualset3
195386	4	415912	7	NULL	NULL	0	NULL	internal standard 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two milliliters of samples containing N-propylprocainamide as the internal standard are buffered to pH 9 and extracted with n-butyl chloride .
	manualset3
195387	5	415912	7	NULL	NULL	0	NULL	pH 9	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two milliliters of samples containing N-propylprocainamide as the internal standard are buffered to pH 9 and extracted with n-butyl chloride .
	manualset3
195388	6	415912	7	NULL	NULL	0	NULL	n-butyl chloride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two milliliters of samples containing N-propylprocainamide as the internal standard are buffered to pH 9 and extracted with n-butyl chloride .
	manualset3
195389	1	415913	7	NULL	NULL	0	NULL	Two models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Two models have provided nonexclusive explanations for the differential effects of LPS and MLA .
	manualset3
195390	2	415913	7	NULL	NULL	0	NULL	nonexclusive explanations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two models have provided nonexclusive explanations for the differential effects of LPS and MLA .
	manualset3
195391	3	415913	7	NULL	NULL	0	NULL	differential effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two models have provided nonexclusive explanations for the differential effects of LPS and MLA .
	manualset3
195392	4	415913	7	NULL	NULL	0	NULL	LPS	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two models have provided nonexclusive explanations for the differential effects of LPS and MLA .
	manualset3
195393	5	415913	7	NULL	NULL	0	NULL	MLA	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two models have provided nonexclusive explanations for the differential effects of LPS and MLA .
	manualset3
195394	1	415914	7	NULL	NULL	0	NULL	Two months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Two months before admission he experienced general illness , fever and itching .
	manualset3
195395	2	415914	7	NULL	NULL	0	NULL	admission	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Two months before admission he experienced general illness , fever and itching .
	manualset3
195396	3	415914	7	NULL	NULL	0	NULL	general illness	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two months before admission he experienced general illness , fever and itching .
	manualset3
195397	4	415914	7	NULL	NULL	0	NULL	fever	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two months before admission he experienced general illness , fever and itching .
	manualset3
195398	5	415914	7	NULL	NULL	NULL	NULL	itching	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two months before admission he experienced general illness , fever and itching .
	manualset3
195399	1	415915	7	NULL	NULL	0	NULL	Two morphologically distinct cell types	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Two morphologically distinct cell types of Coxiella burneti phase I have been separated on the basis of unique buoyant densities .
	manualset3
195400	2	415915	7	NULL	NULL	0	NULL	Coxiella burneti	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two morphologically distinct cell types of Coxiella burneti phase I have been separated on the basis of unique buoyant densities .
	manualset3
195401	3	415915	7	NULL	NULL	0	NULL	phase I	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two morphologically distinct cell types of Coxiella burneti phase I have been separated on the basis of unique buoyant densities .
	manualset3
195402	4	415915	7	NULL	NULL	0	NULL	basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two morphologically distinct cell types of Coxiella burneti phase I have been separated on the basis of unique buoyant densities .
	manualset3
195403	5	415915	7	NULL	NULL	0	NULL	unique buoyant densities	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two morphologically distinct cell types of Coxiella burneti phase I have been separated on the basis of unique buoyant densities .
	manualset3
195404	1	415916	7	NULL	NULL	0	NULL	Two new models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Two new models of chronic serum sickness glomerulonephritis have been developed and characterized , using cationic and native bovine serum albumin ( BSA ) .
	manualset3
195405	2	415916	7	NULL	NULL	0	NULL	chronic serum sickness glomerulonephritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two new models of chronic serum sickness glomerulonephritis have been developed and characterized , using cationic and native bovine serum albumin ( BSA ) .
	manualset3
195406	3	415916	7	NULL	NULL	0	NULL	cationic and native bovine serum albumin ( BSA )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Two new models of chronic serum sickness glomerulonephritis have been developed and characterized , using cationic and native bovine serum albumin ( BSA ) .
	manualset3
195407	1	415917	7	NULL	NULL	0	NULL	Two new types	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Two new types of lentiviral vectors expressing a reporter transgene encoding either firefly luciferase ( fLuc ) for bioluminescence imaging or the HSV1 thymidine kinase ( HSV1-TK ) for radiopharmaceutical-based imaging were constructed to monitor human embryonic stem cell ( hESC ) engraftment and proliferation in live mice after transplantation .
	manualset3
195408	2	415917	7	NULL	NULL	0	NULL	lentiviral vectors	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Two new types of lentiviral vectors expressing a reporter transgene encoding either firefly luciferase ( fLuc ) for bioluminescence imaging or the HSV1 thymidine kinase ( HSV1-TK ) for radiopharmaceutical-based imaging were constructed to monitor human embryonic stem cell ( hESC ) engraftment and proliferation in live mice after transplantation .
	manualset3
195409	3	415917	7	NULL	NULL	0	NULL	reporter transgene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Two new types of lentiviral vectors expressing a reporter transgene encoding either firefly luciferase ( fLuc ) for bioluminescence imaging or the HSV1 thymidine kinase ( HSV1-TK ) for radiopharmaceutical-based imaging were constructed to monitor human embryonic stem cell ( hESC ) engraftment and proliferation in live mice after transplantation .
	manualset3
195410	4	415917	7	NULL	NULL	0	NULL	firefly luciferase ( fLuc )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Two new types of lentiviral vectors expressing a reporter transgene encoding either firefly luciferase ( fLuc ) for bioluminescence imaging or the HSV1 thymidine kinase ( HSV1-TK ) for radiopharmaceutical-based imaging were constructed to monitor human embryonic stem cell ( hESC ) engraftment and proliferation in live mice after transplantation .
	manualset3
195411	5	415917	7	NULL	NULL	0	NULL	bioluminescence imaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two new types of lentiviral vectors expressing a reporter transgene encoding either firefly luciferase ( fLuc ) for bioluminescence imaging or the HSV1 thymidine kinase ( HSV1-TK ) for radiopharmaceutical-based imaging were constructed to monitor human embryonic stem cell ( hESC ) engraftment and proliferation in live mice after transplantation .
	manualset3
195412	6	415917	7	NULL	NULL	0	NULL	HSV1 thymidine kinase ( HSV1-TK ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Two new types of lentiviral vectors expressing a reporter transgene encoding either firefly luciferase ( fLuc ) for bioluminescence imaging or the HSV1 thymidine kinase ( HSV1-TK ) for radiopharmaceutical-based imaging were constructed to monitor human embryonic stem cell ( hESC ) engraftment and proliferation in live mice after transplantation .
	manualset3
195413	7	415917	7	NULL	NULL	0	NULL	radiopharmaceutical-based imaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two new types of lentiviral vectors expressing a reporter transgene encoding either firefly luciferase ( fLuc ) for bioluminescence imaging or the HSV1 thymidine kinase ( HSV1-TK ) for radiopharmaceutical-based imaging were constructed to monitor human embryonic stem cell ( hESC ) engraftment and proliferation in live mice after transplantation .
	manualset3
195414	8	415917	7	NULL	NULL	0	NULL	human embryonic stem cell ( hESC ) engraftment	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two new types of lentiviral vectors expressing a reporter transgene encoding either firefly luciferase ( fLuc ) for bioluminescence imaging or the HSV1 thymidine kinase ( HSV1-TK ) for radiopharmaceutical-based imaging were constructed to monitor human embryonic stem cell ( hESC ) engraftment and proliferation in live mice after transplantation .
	manualset3
195415	9	415917	7	NULL	NULL	0	NULL	human embryonic stem cell ( hESC ) proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two new types of lentiviral vectors expressing a reporter transgene encoding either firefly luciferase ( fLuc ) for bioluminescence imaging or the HSV1 thymidine kinase ( HSV1-TK ) for radiopharmaceutical-based imaging were constructed to monitor human embryonic stem cell ( hESC ) engraftment and proliferation in live mice after transplantation .
	manualset3
195416	10	415917	7	NULL	NULL	0	NULL	live mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two new types of lentiviral vectors expressing a reporter transgene encoding either firefly luciferase ( fLuc ) for bioluminescence imaging or the HSV1 thymidine kinase ( HSV1-TK ) for radiopharmaceutical-based imaging were constructed to monitor human embryonic stem cell ( hESC ) engraftment and proliferation in live mice after transplantation .
	manualset3
195417	11	415917	7	NULL	NULL	0	NULL	transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Two new types of lentiviral vectors expressing a reporter transgene encoding either firefly luciferase ( fLuc ) for bioluminescence imaging or the HSV1 thymidine kinase ( HSV1-TK ) for radiopharmaceutical-based imaging were constructed to monitor human embryonic stem cell ( hESC ) engraftment and proliferation in live mice after transplantation .
	manualset3
195418	1	415918	7	NULL	NULL	NULL	NULL	resuscitation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After resuscitation , a severe metabolic acidosis ( pH 6.65 ) and cardiac dysrrhythmias consistent with sodium channel poisoning were detected .
	manualset3
195419	2	415918	7	NULL	NULL	0	NULL	severe metabolic acidosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	After resuscitation , a severe metabolic acidosis ( pH 6.65 ) and cardiac dysrrhythmias consistent with sodium channel poisoning were detected .
	manualset3
195420	3	415918	7	NULL	NULL	0	NULL	 pH 6.65	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After resuscitation , a severe metabolic acidosis ( pH 6.65 ) and cardiac dysrrhythmias consistent with sodium channel poisoning were detected .
	manualset3
195421	4	415918	7	NULL	NULL	0	NULL	cardiac dysrrhythmias	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	After resuscitation , a severe metabolic acidosis ( pH 6.65 ) and cardiac dysrrhythmias consistent with sodium channel poisoning were detected .
	manualset3
195422	5	415918	7	NULL	NULL	NULL	NULL	sodium channel poisoning	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After resuscitation , a severe metabolic acidosis ( pH 6.65 ) and cardiac dysrrhythmias consistent with sodium channel poisoning were detected .
	manualset3
195423	1	415919	7	NULL	NULL	0	NULL	Two nonidentical , high - affinity cGMP-binding sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Two nonidentical , high - affinity cGMP-binding sites exist on the nonactivated mammalian PDE6R holoenzyme ( alphabetagammagamma ) .
	manualset3
195424	2	415919	7	NULL	NULL	0	NULL	nonactivated mammalian PDE6R holoenzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Two nonidentical , high - affinity cGMP-binding sites exist on the nonactivated mammalian PDE6R holoenzyme ( alphabetagammagamma ) .
	manualset3
195425	3	415919	7	NULL	NULL	0	NULL	alphabetagammagamma 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Two nonidentical , high - affinity cGMP-binding sites exist on the nonactivated mammalian PDE6R holoenzyme ( alphabetagammagamma ) .
	manualset3
195426	1	415920	7	NULL	NULL	0	NULL	Two of the species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two of the species , Aspergillus ochraceoroseus and an undescribed Aspergillus species SRRC 1468 , are morphologically similar to members of Aspergillus section Circumdati .
	manualset3
195427	2	415920	7	NULL	NULL	0	NULL	Aspergillus ochraceoroseus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two of the species , Aspergillus ochraceoroseus and an undescribed Aspergillus species SRRC 1468 , are morphologically similar to members of Aspergillus section Circumdati .
	manualset3
195428	3	415920	7	NULL	NULL	0	NULL	undescribed Aspergillus species SRRC 1468	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two of the species , Aspergillus ochraceoroseus and an undescribed Aspergillus species SRRC 1468 , are morphologically similar to members of Aspergillus section Circumdati .
	manualset3
195429	4	415920	7	NULL	NULL	0	NULL	members	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two of the species , Aspergillus ochraceoroseus and an undescribed Aspergillus species SRRC 1468 , are morphologically similar to members of Aspergillus section Circumdati .
	manualset3
195430	5	415920	7	NULL	NULL	0	NULL	Aspergillus section Circumdati	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two of the species , Aspergillus ochraceoroseus and an undescribed Aspergillus species SRRC 1468 , are morphologically similar to members of Aspergillus section Circumdati .
	manualset3
195431	1	415921	7	NULL	NULL	0	NULL	Two of these reports	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Two of these reports were for deaths , one during surgery and the other as a result of an erosion of the gastric band into the stomach 9 weeks after implantation .
	manualset3
195432	2	415921	7	NULL	NULL	0	NULL	deaths	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two of these reports were for deaths , one during surgery and the other as a result of an erosion of the gastric band into the stomach 9 weeks after implantation .
	manualset3
195433	3	415921	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two of these reports were for deaths , one during surgery and the other as a result of an erosion of the gastric band into the stomach 9 weeks after implantation .
	manualset3
195434	4	415921	7	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Two of these reports were for deaths , one during surgery and the other as a result of an erosion of the gastric band into the stomach 9 weeks after implantation .
	manualset3
195435	5	415921	7	NULL	NULL	0	NULL	 result	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two of these reports were for deaths , one during surgery and the other as a result of an erosion of the gastric band into the stomach 9 weeks after implantation .
	manualset3
195436	6	415921	7	NULL	NULL	0	NULL	erosion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two of these reports were for deaths , one during surgery and the other as a result of an erosion of the gastric band into the stomach 9 weeks after implantation .
	manualset3
195437	7	415921	7	NULL	NULL	0	NULL	gastric band	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two of these reports were for deaths , one during surgery and the other as a result of an erosion of the gastric band into the stomach 9 weeks after implantation .
	manualset3
195438	8	415921	7	NULL	NULL	0	NULL	stomach	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Two of these reports were for deaths , one during surgery and the other as a result of an erosion of the gastric band into the stomach 9 weeks after implantation .
	manualset3
195439	9	415921	7	NULL	NULL	0	NULL	9 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Two of these reports were for deaths , one during surgery and the other as a result of an erosion of the gastric band into the stomach 9 weeks after implantation .
	manualset3
195440	10	415921	7	NULL	NULL	0	NULL	implantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Two of these reports were for deaths , one during surgery and the other as a result of an erosion of the gastric band into the stomach 9 weeks after implantation .
	manualset3
195441	1	415922	7	NULL	NULL	0	NULL	Two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two of these required subsequent repeat ACS 6 and 9 months later with one patient eventually requiring tracheostomy .
	manualset3
195442	2	415922	7	NULL	NULL	0	NULL	 subsequent repeat ACS 6 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Two of these required subsequent repeat ACS 6 and 9 months later with one patient eventually requiring tracheostomy .
	manualset3
195443	3	415922	7	NULL	NULL	0	NULL	 subsequent repeat ACS 9 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Two of these required subsequent repeat ACS 6 and 9 months later with one patient eventually requiring tracheostomy .
	manualset3
195444	4	415922	7	NULL	NULL	0	NULL	one patient	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two of these required subsequent repeat ACS 6 and 9 months later with one patient eventually requiring tracheostomy .
	manualset3
195445	5	415922	7	NULL	NULL	0	NULL	tracheostomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Two of these required subsequent repeat ACS 6 and 9 months later with one patient eventually requiring tracheostomy .
	manualset3
195446	1	415923	7	NULL	NULL	0	NULL	Two or more epithelial ovarian cancers 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two or more epithelial ovarian cancers in close relatives , or ovarian cancer in conjunction with young-onset breast or colonic cancers , are suggestive of an inherited predisposition .
	manualset3
195447	2	415923	7	NULL	NULL	0	NULL	close relatives	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Two or more epithelial ovarian cancers in close relatives , or ovarian cancer in conjunction with young-onset breast or colonic cancers , are suggestive of an inherited predisposition .
	manualset3
195448	3	415923	7	NULL	NULL	0	NULL	ovarian cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two or more epithelial ovarian cancers in close relatives , or ovarian cancer in conjunction with young-onset breast or colonic cancers , are suggestive of an inherited predisposition .
	manualset3
195449	4	415923	7	NULL	NULL	0	NULL	conjunction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two or more epithelial ovarian cancers in close relatives , or ovarian cancer in conjunction with young-onset breast or colonic cancers , are suggestive of an inherited predisposition .
	manualset3
195450	5	415923	7	NULL	NULL	0	NULL	young-onset breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two or more epithelial ovarian cancers in close relatives , or ovarian cancer in conjunction with young-onset breast or colonic cancers , are suggestive of an inherited predisposition .
	manualset3
195451	6	415923	7	NULL	NULL	0	NULL	 young-onset colonic cancers	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two or more epithelial ovarian cancers in close relatives , or ovarian cancer in conjunction with young-onset breast or colonic cancers , are suggestive of an inherited predisposition .
	manualset3
195452	7	415923	7	NULL	NULL	NULL	NULL	inherited predisposition	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two or more epithelial ovarian cancers in close relatives , or ovarian cancer in conjunction with young-onset breast or colonic cancers , are suggestive of an inherited predisposition .
	manualset3
195468	1	415924	7	NULL	NULL	0	NULL	Two other mutants	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two other mutants showed activity on p-nitrophenyl -- d-glucopyranoside , which showed no activity at all with the wild type enzyme .
	manualset3
195469	2	415924	7	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two other mutants showed activity on p-nitrophenyl -- d-glucopyranoside , which showed no activity at all with the wild type enzyme .
	manualset3
195471	3	415924	7	NULL	NULL	0	NULL	 p-nitrophenyl -- d-glucopyranoside	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two other mutants showed activity on p-nitrophenyl -- d-glucopyranoside , which showed no activity at all with the wild type enzyme .
	manualset3
195476	4	415924	7	NULL	NULL	0	NULL	no activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two other mutants showed activity on p-nitrophenyl -- d-glucopyranoside , which showed no activity at all with the wild type enzyme .
	manualset3
195478	5	415924	7	NULL	NULL	0	NULL	wild type enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Two other mutants showed activity on p-nitrophenyl -- d-glucopyranoside , which showed no activity at all with the wild type enzyme .
	manualset3
195483	1	415925	7	NULL	NULL	0	NULL	Two pairs 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two pairs of expanded granular sludge bed ( EGSB ) bioreactors , R1/R2 and R3/R4 , were designed .
	manualset3
195485	2	415925	7	NULL	NULL	0	NULL	expanded granular sludge bed ( EGSB ) bioreactors	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Two pairs of expanded granular sludge bed ( EGSB ) bioreactors , R1/R2 and R3/R4 , were designed .
	manualset3
195487	3	415925	7	NULL	NULL	0	NULL	R1/R2	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Two pairs of expanded granular sludge bed ( EGSB ) bioreactors , R1/R2 and R3/R4 , were designed .
	manualset3
195488	4	415925	7	NULL	NULL	0	NULL	R3/R4	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Two pairs of expanded granular sludge bed ( EGSB ) bioreactors , R1/R2 and R3/R4 , were designed .
	manualset3
195489	1	415926	7	NULL	NULL	0	NULL	Two part collectives	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two part collectives of patients with carcinomas of the uterus - one consisting of 525 conventionally irradiated patients , the other consisting of 577 patients irradiated with telecobalt - are compared with respect to their five-year survival recovery rate , the frequency of recurrences and metastases and the radiogenic complications .
	manualset3
195490	2	415926	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two part collectives of patients with carcinomas of the uterus - one consisting of 525 conventionally irradiated patients , the other consisting of 577 patients irradiated with telecobalt - are compared with respect to their five-year survival recovery rate , the frequency of recurrences and metastases and the radiogenic complications .
	manualset3
195491	3	415926	7	NULL	NULL	0	NULL	carcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two part collectives of patients with carcinomas of the uterus - one consisting of 525 conventionally irradiated patients , the other consisting of 577 patients irradiated with telecobalt - are compared with respect to their five-year survival recovery rate , the frequency of recurrences and metastases and the radiogenic complications .
	manualset3
195492	4	415926	7	NULL	NULL	0	NULL	uterus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Two part collectives of patients with carcinomas of the uterus - one consisting of 525 conventionally irradiated patients , the other consisting of 577 patients irradiated with telecobalt - are compared with respect to their five-year survival recovery rate , the frequency of recurrences and metastases and the radiogenic complications .
	manualset3
195493	5	415926	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two part collectives of patients with carcinomas of the uterus - one consisting of 525 conventionally irradiated patients , the other consisting of 577 patients irradiated with telecobalt - are compared with respect to their five-year survival recovery rate , the frequency of recurrences and metastases and the radiogenic complications .
	manualset3
195495	7	415926	7	NULL	NULL	NULL	NULL	525 conventionally irradiated patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two part collectives of patients with carcinomas of the uterus - one consisting of 525 conventionally irradiated patients , the other consisting of 577 patients irradiated with telecobalt - are compared with respect to their five-year survival recovery rate , the frequency of recurrences and metastases and the radiogenic complications .
	manualset3
195502	8	415926	7	NULL	NULL	0	NULL	577 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two part collectives of patients with carcinomas of the uterus - one consisting of 525 conventionally irradiated patients , the other consisting of 577 patients irradiated with telecobalt - are compared with respect to their five-year survival recovery rate , the frequency of recurrences and metastases and the radiogenic complications .
	manualset3
195503	9	415926	7	NULL	NULL	0	NULL	telecobalt	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two part collectives of patients with carcinomas of the uterus - one consisting of 525 conventionally irradiated patients , the other consisting of 577 patients irradiated with telecobalt - are compared with respect to their five-year survival recovery rate , the frequency of recurrences and metastases and the radiogenic complications .
	manualset3
195506	10	415926	7	NULL	NULL	0	NULL	 five-year survival recovery rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two part collectives of patients with carcinomas of the uterus - one consisting of 525 conventionally irradiated patients , the other consisting of 577 patients irradiated with telecobalt - are compared with respect to their five-year survival recovery rate , the frequency of recurrences and metastases and the radiogenic complications .
	manualset3
195511	11	415926	7	NULL	NULL	0	NULL	frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two part collectives of patients with carcinomas of the uterus - one consisting of 525 conventionally irradiated patients , the other consisting of 577 patients irradiated with telecobalt - are compared with respect to their five-year survival recovery rate , the frequency of recurrences and metastases and the radiogenic complications .
	manualset3
195512	12	415926	7	NULL	NULL	0	NULL	recurrences	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two part collectives of patients with carcinomas of the uterus - one consisting of 525 conventionally irradiated patients , the other consisting of 577 patients irradiated with telecobalt - are compared with respect to their five-year survival recovery rate , the frequency of recurrences and metastases and the radiogenic complications .
	manualset3
195513	13	415926	7	NULL	NULL	0	NULL	metastases	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two part collectives of patients with carcinomas of the uterus - one consisting of 525 conventionally irradiated patients , the other consisting of 577 patients irradiated with telecobalt - are compared with respect to their five-year survival recovery rate , the frequency of recurrences and metastases and the radiogenic complications .
	manualset3
195514	14	415926	7	NULL	NULL	0	NULL	radiogenic complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two part collectives of patients with carcinomas of the uterus - one consisting of 525 conventionally irradiated patients , the other consisting of 577 patients irradiated with telecobalt - are compared with respect to their five-year survival recovery rate , the frequency of recurrences and metastases and the radiogenic complications .
	manualset3
195515	1	415927	7	NULL	NULL	0	NULL	Two patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients presented with pulmonary infiltrates and one with a hepatic tumor .
	manualset3
195516	2	415927	7	NULL	NULL	0	NULL	pulmonary infiltrates	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients presented with pulmonary infiltrates and one with a hepatic tumor .
	manualset3
195517	3	415927	7	NULL	NULL	0	NULL	one	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients presented with pulmonary infiltrates and one with a hepatic tumor .
	manualset3
195518	4	415927	7	NULL	NULL	0	NULL	hepatic tumor	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients presented with pulmonary infiltrates and one with a hepatic tumor .
	manualset3
195519	1	415928	7	NULL	NULL	0	NULL	Two patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients were at nine and 15 weeks of gestation and postoperatively were well following termination of pregnancy .
	manualset3
195521	2	415928	7	NULL	NULL	0	NULL	nine weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients were at nine and 15 weeks of gestation and postoperatively were well following termination of pregnancy .
	manualset3
195523	3	415928	7	NULL	NULL	0	NULL	15 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients were at nine and 15 weeks of gestation and postoperatively were well following termination of pregnancy .
	manualset3
195526	4	415928	7	NULL	NULL	0	NULL	gestation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients were at nine and 15 weeks of gestation and postoperatively were well following termination of pregnancy .
	manualset3
195528	5	415928	7	NULL	NULL	0	NULL	termination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients were at nine and 15 weeks of gestation and postoperatively were well following termination of pregnancy .
	manualset3
195533	6	415928	7	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients were at nine and 15 weeks of gestation and postoperatively were well following termination of pregnancy .
	manualset3
195534	1	415929	7	NULL	NULL	0	NULL	Two patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients were followed for a year and have had return of psychiatric symptoms or facial pain ; both have been maintained on medication and have returned to normal activities .
	manualset3
195535	2	415929	7	NULL	NULL	0	NULL	year	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients were followed for a year and have had return of psychiatric symptoms or facial pain ; both have been maintained on medication and have returned to normal activities .
	manualset3
195536	3	415929	7	NULL	NULL	0	NULL	return	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients were followed for a year and have had return of psychiatric symptoms or facial pain ; both have been maintained on medication and have returned to normal activities .
	manualset3
195537	4	415929	7	NULL	NULL	0	NULL	psychiatric symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients were followed for a year and have had return of psychiatric symptoms or facial pain ; both have been maintained on medication and have returned to normal activities .
	manualset3
195538	5	415929	7	NULL	NULL	0	NULL	facial pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients were followed for a year and have had return of psychiatric symptoms or facial pain ; both have been maintained on medication and have returned to normal activities .
	manualset3
195539	6	415929	7	NULL	NULL	0	NULL	medication	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients were followed for a year and have had return of psychiatric symptoms or facial pain ; both have been maintained on medication and have returned to normal activities .
	manualset3
195540	7	415929	7	NULL	NULL	0	NULL	 normal activities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients were followed for a year and have had return of psychiatric symptoms or facial pain ; both have been maintained on medication and have returned to normal activities .
	manualset3
195541	1	415930	7	NULL	NULL	NULL	NULL	reviewing the literature	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After reviewing the literature on sex offenders-a literature largely devoted to behavioral , cognitive-behavioral , and relapse-prevention approaches to treatment-the author proposes that an object-relational group psychotherapy treatment has a great deal to offer in the treatment of incest offenders .
	manualset3
195542	2	415930	7	NULL	NULL	0	NULL	sex offenders	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	After reviewing the literature on sex offenders-a literature largely devoted to behavioral , cognitive-behavioral , and relapse-prevention approaches to treatment-the author proposes that an object-relational group psychotherapy treatment has a great deal to offer in the treatment of incest offenders .
	manualset3
195543	3	415930	7	NULL	NULL	0	NULL	literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	After reviewing the literature on sex offenders-a literature largely devoted to behavioral , cognitive-behavioral , and relapse-prevention approaches to treatment-the author proposes that an object-relational group psychotherapy treatment has a great deal to offer in the treatment of incest offenders .
	manualset3
195544	4	415930	7	NULL	NULL	NULL	NULL	behavioral approaches	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After reviewing the literature on sex offenders-a literature largely devoted to behavioral , cognitive-behavioral , and relapse-prevention approaches to treatment-the author proposes that an object-relational group psychotherapy treatment has a great deal to offer in the treatment of incest offenders .
	manualset3
195545	5	415930	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After reviewing the literature on sex offenders-a literature largely devoted to behavioral , cognitive-behavioral , and relapse-prevention approaches to treatment-the author proposes that an object-relational group psychotherapy treatment has a great deal to offer in the treatment of incest offenders .
	manualset3
195546	6	415930	7	NULL	NULL	0	NULL	author	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	After reviewing the literature on sex offenders-a literature largely devoted to behavioral , cognitive-behavioral , and relapse-prevention approaches to treatment-the author proposes that an object-relational group psychotherapy treatment has a great deal to offer in the treatment of incest offenders .
	manualset3
195547	7	415930	7	NULL	NULL	0	NULL	object-relational group psychotherapy treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After reviewing the literature on sex offenders-a literature largely devoted to behavioral , cognitive-behavioral , and relapse-prevention approaches to treatment-the author proposes that an object-relational group psychotherapy treatment has a great deal to offer in the treatment of incest offenders .
	manualset3
195548	8	415930	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After reviewing the literature on sex offenders-a literature largely devoted to behavioral , cognitive-behavioral , and relapse-prevention approaches to treatment-the author proposes that an object-relational group psychotherapy treatment has a great deal to offer in the treatment of incest offenders .
	manualset3
195549	9	415930	7	NULL	NULL	0	NULL	 incest offenders	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	After reviewing the literature on sex offenders-a literature largely devoted to behavioral , cognitive-behavioral , and relapse-prevention approaches to treatment-the author proposes that an object-relational group psychotherapy treatment has a great deal to offer in the treatment of incest offenders .
	manualset3
197257	10	415930	7	NULL	NULL	0	NULL	 cognitive-behavioral approaches	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After reviewing the literature on sex offenders-a literature largely devoted to behavioral , cognitive-behavioral , and relapse-prevention approaches to treatment-the author proposes that an object-relational group psychotherapy treatment has a great deal to offer in the treatment of incest offenders .
	manualset3
197258	11	415930	7	NULL	NULL	0	NULL	 relapse-prevention approaches	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After reviewing the literature on sex offenders-a literature largely devoted to behavioral , cognitive-behavioral , and relapse-prevention approaches to treatment-the author proposes that an object-relational group psychotherapy treatment has a great deal to offer in the treatment of incest offenders .
	manualset3
195554	1	415931	7	NULL	NULL	0	NULL	Two patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients with PR were able to undergo complete surgical resection , making the overall rate of complete response , including surgery , 73 % .
	manualset3
195555	2	415931	7	NULL	NULL	0	NULL	PR	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients with PR were able to undergo complete surgical resection , making the overall rate of complete response , including surgery , 73 % .
	manualset3
195556	3	415931	7	NULL	NULL	0	NULL	complete surgical resection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients with PR were able to undergo complete surgical resection , making the overall rate of complete response , including surgery , 73 % .
	manualset3
195557	4	415931	7	NULL	NULL	0	NULL	overall rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients with PR were able to undergo complete surgical resection , making the overall rate of complete response , including surgery , 73 % .
	manualset3
195558	5	415931	7	NULL	NULL	0	NULL	complete response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients with PR were able to undergo complete surgical resection , making the overall rate of complete response , including surgery , 73 % .
	manualset3
195559	6	415931	7	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients with PR were able to undergo complete surgical resection , making the overall rate of complete response , including surgery , 73 % .
	manualset3
195560	7	415931	7	NULL	NULL	0	NULL	73 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients with PR were able to undergo complete surgical resection , making the overall rate of complete response , including surgery , 73 % .
	manualset3
195741	1	415932	7	NULL	NULL	0	NULL	Two patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients with acute leukemia developed PTR after allogeneic BMT from one HLA-antigen-mismatched mother attributable to HLA antibodies , which could not be detected in their serum before BMT .
	manualset3
195742	2	415932	7	NULL	NULL	0	NULL	acute leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients with acute leukemia developed PTR after allogeneic BMT from one HLA-antigen-mismatched mother attributable to HLA antibodies , which could not be detected in their serum before BMT .
	manualset3
195743	3	415932	7	NULL	NULL	0	NULL	PTR	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients with acute leukemia developed PTR after allogeneic BMT from one HLA-antigen-mismatched mother attributable to HLA antibodies , which could not be detected in their serum before BMT .
	manualset3
195744	4	415932	7	NULL	NULL	0	NULL	allogeneic BMT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients with acute leukemia developed PTR after allogeneic BMT from one HLA-antigen-mismatched mother attributable to HLA antibodies , which could not be detected in their serum before BMT .
	manualset3
195745	5	415932	7	NULL	NULL	0	NULL	one HLA-antigen-mismatched mother	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients with acute leukemia developed PTR after allogeneic BMT from one HLA-antigen-mismatched mother attributable to HLA antibodies , which could not be detected in their serum before BMT .
	manualset3
195746	6	415932	7	NULL	NULL	0	NULL	HLA antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients with acute leukemia developed PTR after allogeneic BMT from one HLA-antigen-mismatched mother attributable to HLA antibodies , which could not be detected in their serum before BMT .
	manualset3
195747	7	415932	7	NULL	NULL	0	NULL	serum 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients with acute leukemia developed PTR after allogeneic BMT from one HLA-antigen-mismatched mother attributable to HLA antibodies , which could not be detected in their serum before BMT .
	manualset3
195748	8	415932	7	NULL	NULL	0	NULL	 BMT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients with acute leukemia developed PTR after allogeneic BMT from one HLA-antigen-mismatched mother attributable to HLA antibodies , which could not be detected in their serum before BMT .
	manualset3
195749	1	415933	7	NULL	NULL	0	NULL	Two patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients with mini-volcano type of skin lesions which showed histopathologic features of cutaneous leishmaniasis ( CL ) have been described .
	manualset3
195750	2	415933	7	NULL	NULL	0	NULL	mini-volcano type	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients with mini-volcano type of skin lesions which showed histopathologic features of cutaneous leishmaniasis ( CL ) have been described .
	manualset3
195751	3	415933	7	NULL	NULL	0	NULL	skin lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients with mini-volcano type of skin lesions which showed histopathologic features of cutaneous leishmaniasis ( CL ) have been described .
	manualset3
195752	4	415933	7	NULL	NULL	0	NULL	histopathologic features	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients with mini-volcano type of skin lesions which showed histopathologic features of cutaneous leishmaniasis ( CL ) have been described .
	manualset3
195753	5	415933	7	NULL	NULL	0	NULL	cutaneous leishmaniasis ( CL )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients with mini-volcano type of skin lesions which showed histopathologic features of cutaneous leishmaniasis ( CL ) have been described .
	manualset3
195754	1	415934	7	NULL	NULL	0	NULL	Two populations	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Two populations of muscles , isolated from the rabbit right ventricle , have been previously described and distinguished on the basis of the presence or absence of transverse ( T ) tubules .
	manualset3
195755	2	415934	7	NULL	NULL	0	NULL	muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Two populations of muscles , isolated from the rabbit right ventricle , have been previously described and distinguished on the basis of the presence or absence of transverse ( T ) tubules .
	manualset3
195756	3	415934	7	NULL	NULL	0	NULL	rabbit right ventricle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Two populations of muscles , isolated from the rabbit right ventricle , have been previously described and distinguished on the basis of the presence or absence of transverse ( T ) tubules .
	manualset3
195757	4	415934	7	NULL	NULL	0	NULL	basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two populations of muscles , isolated from the rabbit right ventricle , have been previously described and distinguished on the basis of the presence or absence of transverse ( T ) tubules .
	manualset3
195758	5	415934	7	NULL	NULL	0	NULL	transverse ( T ) tubules	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Two populations of muscles , isolated from the rabbit right ventricle , have been previously described and distinguished on the basis of the presence or absence of transverse ( T ) tubules .
	manualset3
195759	1	415935	7	NULL	NULL	NULL	NULL	Two premature stop codons	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two premature stop codons , Ser346ter and Tyr415ter , were identified in germ-line RAD52 alleles from 5 % of early-onset breast cancer cases .
	manualset3
195760	2	415935	7	NULL	NULL	0	NULL	Ser346ter	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Two premature stop codons , Ser346ter and Tyr415ter , were identified in germ-line RAD52 alleles from 5 % of early-onset breast cancer cases .
	manualset3
195761	3	415935	7	NULL	NULL	0	NULL	Tyr415ter	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Two premature stop codons , Ser346ter and Tyr415ter , were identified in germ-line RAD52 alleles from 5 % of early-onset breast cancer cases .
	manualset3
195762	4	415935	7	NULL	NULL	0	NULL	germ-line RAD52 alleles	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Two premature stop codons , Ser346ter and Tyr415ter , were identified in germ-line RAD52 alleles from 5 % of early-onset breast cancer cases .
	manualset3
195763	5	415935	7	NULL	NULL	0	NULL	5 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two premature stop codons , Ser346ter and Tyr415ter , were identified in germ-line RAD52 alleles from 5 % of early-onset breast cancer cases .
	manualset3
195764	6	415935	7	NULL	NULL	0	NULL	early-onset breast cancer cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two premature stop codons , Ser346ter and Tyr415ter , were identified in germ-line RAD52 alleles from 5 % of early-onset breast cancer cases .
	manualset3
195765	1	415936	7	NULL	NULL	0	NULL	Two proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two proteins ( M.W. 98 , 000 and 31 , 000 ) were significantly alkylated by ( 3H ) N-ethylmaleimide and protected by phosphate and nigericin .
	manualset3
195766	2	415936	7	NULL	NULL	0	NULL	M.W. 98 , 000	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two proteins ( M.W. 98 , 000 and 31 , 000 ) were significantly alkylated by ( 3H ) N-ethylmaleimide and protected by phosphate and nigericin .
	manualset3
195767	3	415936	7	NULL	NULL	0	NULL	M.W. 31 , 000	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two proteins ( M.W. 98 , 000 and 31 , 000 ) were significantly alkylated by ( 3H ) N-ethylmaleimide and protected by phosphate and nigericin .
	manualset3
195768	4	415936	7	NULL	NULL	0	NULL	( 3H ) N-ethylmaleimide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two proteins ( M.W. 98 , 000 and 31 , 000 ) were significantly alkylated by ( 3H ) N-ethylmaleimide and protected by phosphate and nigericin .
	manualset3
195769	5	415936	7	NULL	NULL	0	NULL	phosphate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two proteins ( M.W. 98 , 000 and 31 , 000 ) were significantly alkylated by ( 3H ) N-ethylmaleimide and protected by phosphate and nigericin .
	manualset3
195770	6	415936	7	NULL	NULL	0	NULL	nigericin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Two proteins ( M.W. 98 , 000 and 31 , 000 ) were significantly alkylated by ( 3H ) N-ethylmaleimide and protected by phosphate and nigericin .
	manualset3
195771	1	415937	7	NULL	NULL	0	NULL	Two proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two proteins , named PMIS1 and PMIS2 , were missing in spermatozoa from Clgn-disrupted mice .
	manualset3
195772	2	415937	7	NULL	NULL	0	NULL	PMIS1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Two proteins , named PMIS1 and PMIS2 , were missing in spermatozoa from Clgn-disrupted mice .
	manualset3
195773	3	415937	7	NULL	NULL	0	NULL	PMIS2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Two proteins , named PMIS1 and PMIS2 , were missing in spermatozoa from Clgn-disrupted mice .
	manualset3
195774	4	415937	7	NULL	NULL	0	NULL	spermatozoa	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Two proteins , named PMIS1 and PMIS2 , were missing in spermatozoa from Clgn-disrupted mice .
	manualset3
195775	5	415937	7	NULL	NULL	0	NULL	Clgn-disrupted mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two proteins , named PMIS1 and PMIS2 , were missing in spermatozoa from Clgn-disrupted mice .
	manualset3
195776	1	415938	7	NULL	NULL	0	NULL	Two proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two proteins specific for lung stem cells/progenitors responsible for local tissue repair were also compared .
	manualset3
195777	2	415938	7	NULL	NULL	0	NULL	lung stem cells/progenitors	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Two proteins specific for lung stem cells/progenitors responsible for local tissue repair were also compared .
	manualset3
195778	3	415938	7	NULL	NULL	0	NULL	local tissue repair 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two proteins specific for lung stem cells/progenitors responsible for local tissue repair were also compared .
	manualset3
195779	1	415939	7	NULL	NULL	0	NULL	Two rat liver cDNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Two rat liver cDNAs encoding CTP : phosphocholine cytidylyltransferase ( CT-1 and CT-2 ) were expressed in COS cells .
	manualset3
195780	2	415939	7	NULL	NULL	0	NULL	CTP : phosphocholine cytidylyltransferase ( CT-1 and CT-2 )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two rat liver cDNAs encoding CTP : phosphocholine cytidylyltransferase ( CT-1 and CT-2 ) were expressed in COS cells .
	manualset3
195781	3	415939	7	NULL	NULL	0	NULL	COS cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Two rat liver cDNAs encoding CTP : phosphocholine cytidylyltransferase ( CT-1 and CT-2 ) were expressed in COS cells .
	manualset3
195782	1	415940	7	NULL	NULL	0	NULL	Two regions 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Two regions of homology exist for the predicted amino acid sequence in common with chromogranin-A and B proteins , a zinc finger protein , and the ryanodine receptor .
	manualset3
195783	2	415940	7	NULL	NULL	0	NULL	homology	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Two regions of homology exist for the predicted amino acid sequence in common with chromogranin-A and B proteins , a zinc finger protein , and the ryanodine receptor .
	manualset3
195784	3	415940	7	NULL	NULL	0	NULL	amino acid sequence	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Two regions of homology exist for the predicted amino acid sequence in common with chromogranin-A and B proteins , a zinc finger protein , and the ryanodine receptor .
	manualset3
195785	4	415940	7	NULL	NULL	NULL	NULL	chromogranin-A proteins	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two regions of homology exist for the predicted amino acid sequence in common with chromogranin-A and B proteins , a zinc finger protein , and the ryanodine receptor .
	manualset3
195786	5	415940	7	NULL	NULL	NULL	NULL	chromogranin-B proteins	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two regions of homology exist for the predicted amino acid sequence in common with chromogranin-A and B proteins , a zinc finger protein , and the ryanodine receptor .
	manualset3
195787	6	415940	7	NULL	NULL	0	NULL	zinc finger protein	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two regions of homology exist for the predicted amino acid sequence in common with chromogranin-A and B proteins , a zinc finger protein , and the ryanodine receptor .
	manualset3
195788	7	415940	7	NULL	NULL	0	NULL	ryanodine receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Two regions of homology exist for the predicted amino acid sequence in common with chromogranin-A and B proteins , a zinc finger protein , and the ryanodine receptor .
	manualset3
195789	1	415941	7	NULL	NULL	0	NULL	Two satellite images	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two satellite images are examined in time series over the 13 years following the founding of the sanctuary through a cross-tabulation technique of dominant classes of vegetation density .
	manualset3
195790	2	415941	7	NULL	NULL	0	NULL	time series	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Two satellite images are examined in time series over the 13 years following the founding of the sanctuary through a cross-tabulation technique of dominant classes of vegetation density .
	manualset3
195791	3	415941	7	NULL	NULL	0	NULL	13 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Two satellite images are examined in time series over the 13 years following the founding of the sanctuary through a cross-tabulation technique of dominant classes of vegetation density .
	manualset3
195792	4	415941	7	NULL	NULL	0	NULL	sanctuary	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Two satellite images are examined in time series over the 13 years following the founding of the sanctuary through a cross-tabulation technique of dominant classes of vegetation density .
	manualset3
195793	5	415941	7	NULL	NULL	0	NULL	cross-tabulation technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two satellite images are examined in time series over the 13 years following the founding of the sanctuary through a cross-tabulation technique of dominant classes of vegetation density .
	manualset3
195794	6	415941	7	NULL	NULL	0	NULL	dominant classes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two satellite images are examined in time series over the 13 years following the founding of the sanctuary through a cross-tabulation technique of dominant classes of vegetation density .
	manualset3
195795	7	415941	7	NULL	NULL	NULL	NULL	vegetation density	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two satellite images are examined in time series over the 13 years following the founding of the sanctuary through a cross-tabulation technique of dominant classes of vegetation density .
	manualset3
195796	1	415942	7	NULL	NULL	0	NULL	Two schools	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Two schools picked for pilot have ties to NCHL board .
	manualset3
195797	2	415942	7	NULL	NULL	0	NULL	pilot	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two schools picked for pilot have ties to NCHL board .
	manualset3
195798	3	415942	7	NULL	NULL	0	NULL	 NCHL board	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Two schools picked for pilot have ties to NCHL board .
	manualset3
195799	1	415943	7	NULL	NULL	0	NULL	Two separate requirements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two separate requirements must be met for categorical perception : ( a ) Discrimination performance must be phonetically mediated ( i.e. , it should be predictable from labeling performance ) , ( b ) labeling responses must be independent of the stimulus context .
	manualset3
195800	2	415943	7	NULL	NULL	0	NULL	categorical perception	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two separate requirements must be met for categorical perception : ( a ) Discrimination performance must be phonetically mediated ( i.e. , it should be predictable from labeling performance ) , ( b ) labeling responses must be independent of the stimulus context .
	manualset3
195801	3	415943	7	NULL	NULL	0	NULL	Discrimination performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two separate requirements must be met for categorical perception : ( a ) Discrimination performance must be phonetically mediated ( i.e. , it should be predictable from labeling performance ) , ( b ) labeling responses must be independent of the stimulus context .
	manualset3
195803	5	415943	7	NULL	NULL	0	NULL	labeling performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two separate requirements must be met for categorical perception : ( a ) Discrimination performance must be phonetically mediated ( i.e. , it should be predictable from labeling performance ) , ( b ) labeling responses must be independent of the stimulus context .
	manualset3
195804	6	415943	7	NULL	NULL	0	NULL	labeling responses	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two separate requirements must be met for categorical perception : ( a ) Discrimination performance must be phonetically mediated ( i.e. , it should be predictable from labeling performance ) , ( b ) labeling responses must be independent of the stimulus context .
	manualset3
195805	7	415943	7	NULL	NULL	0	NULL	stimulus context	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two separate requirements must be met for categorical perception : ( a ) Discrimination performance must be phonetically mediated ( i.e. , it should be predictable from labeling performance ) , ( b ) labeling responses must be independent of the stimulus context .
	manualset3
195806	1	415944	7	NULL	NULL	0	NULL	Two sequential s.c. injections	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Two sequential s.c. injections of oestrone sulphate enhanced the enzyme activities significantly in liver and white blood cells , but not in spleen .
	manualset3
195807	2	415944	7	NULL	NULL	NULL	NULL	oestrone sulphate 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two sequential s.c. injections of oestrone sulphate enhanced the enzyme activities significantly in liver and white blood cells , but not in spleen .
	manualset3
195808	3	415944	7	NULL	NULL	0	NULL	enzyme activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two sequential s.c. injections of oestrone sulphate enhanced the enzyme activities significantly in liver and white blood cells , but not in spleen .
	manualset3
195809	4	415944	7	NULL	NULL	0	NULL	liver cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Two sequential s.c. injections of oestrone sulphate enhanced the enzyme activities significantly in liver and white blood cells , but not in spleen .
	manualset3
195810	5	415944	7	NULL	NULL	0	NULL	white blood cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Two sequential s.c. injections of oestrone sulphate enhanced the enzyme activities significantly in liver and white blood cells , but not in spleen .
	manualset3
195811	6	415944	7	NULL	NULL	0	NULL	spleen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Two sequential s.c. injections of oestrone sulphate enhanced the enzyme activities significantly in liver and white blood cells , but not in spleen .
	manualset3
195812	1	415945	7	NULL	NULL	NULL	NULL	scaling and root planing	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After scaling and root planing , each selected site was randomly assigned to one of two treatment groups : tetracycline fiber therapy and control group .
	manualset3
195813	2	415945	7	NULL	NULL	0	NULL	selected site 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After scaling and root planing , each selected site was randomly assigned to one of two treatment groups : tetracycline fiber therapy and control group .
	manualset3
195814	3	415945	7	NULL	NULL	0	NULL	one of two treatment groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	After scaling and root planing , each selected site was randomly assigned to one of two treatment groups : tetracycline fiber therapy and control group .
	manualset3
195815	4	415945	7	NULL	NULL	NULL	NULL	tetracycline fiber therapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After scaling and root planing , each selected site was randomly assigned to one of two treatment groups : tetracycline fiber therapy and control group .
	manualset3
195816	5	415945	7	NULL	NULL	0	NULL	control group 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	After scaling and root planing , each selected site was randomly assigned to one of two treatment groups : tetracycline fiber therapy and control group .
	manualset3
195817	1	415946	7	NULL	NULL	0	NULL	Two sets	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two sets of mutations : the Q151 M complex and the 69 insert , cause resistance to multiple nucleoside analogs .
	manualset3
195818	2	415946	7	NULL	NULL	0	NULL	mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two sets of mutations : the Q151 M complex and the 69 insert , cause resistance to multiple nucleoside analogs .
	manualset3
195819	3	415946	7	NULL	NULL	0	NULL	 Q151 M complex	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Two sets of mutations : the Q151 M complex and the 69 insert , cause resistance to multiple nucleoside analogs .
	manualset3
195820	4	415946	7	NULL	NULL	0	NULL	 69 insert	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Two sets of mutations : the Q151 M complex and the 69 insert , cause resistance to multiple nucleoside analogs .
	manualset3
195821	5	415946	7	NULL	NULL	0	NULL	 resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two sets of mutations : the Q151 M complex and the 69 insert , cause resistance to multiple nucleoside analogs .
	manualset3
195822	6	415946	7	NULL	NULL	0	NULL	multiple nucleoside analogs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two sets of mutations : the Q151 M complex and the 69 insert , cause resistance to multiple nucleoside analogs .
	manualset3
195823	1	415947	7	NULL	NULL	0	NULL	Two severe cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two severe cases of rhabdomyolysis occurred .
	manualset3
195824	2	415947	7	NULL	NULL	0	NULL	rhabdomyolysis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two severe cases of rhabdomyolysis occurred .
	manualset3
195825	1	415948	7	NULL	NULL	0	NULL	Two sides	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two sides to every story : the HIF-dependent and HIF-independent functions of pVHL .
	manualset3
195826	2	415948	7	NULL	NULL	0	NULL	every story	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two sides to every story : the HIF-dependent and HIF-independent functions of pVHL .
	manualset3
195827	3	415948	7	NULL	NULL	0	NULL	 HIF-dependent functions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two sides to every story : the HIF-dependent and HIF-independent functions of pVHL .
	manualset3
195828	4	415948	7	NULL	NULL	0	NULL	HIF-independent functions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two sides to every story : the HIF-dependent and HIF-independent functions of pVHL .
	manualset3
195829	5	415948	7	NULL	NULL	0	NULL	 pVHL	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two sides to every story : the HIF-dependent and HIF-independent functions of pVHL .
	manualset3
195830	1	415949	7	NULL	NULL	0	NULL	Two species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two species , Clethrionomys glareolus and Apodemus agrarius , were found positive for hantaviral antigen in 13.7 % and 4.5 % of the investigated rodents , respectively .
	manualset3
195831	2	415949	7	NULL	NULL	0	NULL	Clethrionomys glareolus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two species , Clethrionomys glareolus and Apodemus agrarius , were found positive for hantaviral antigen in 13.7 % and 4.5 % of the investigated rodents , respectively .
	manualset3
195832	3	415949	7	NULL	NULL	0	NULL	Apodemus agrarius	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two species , Clethrionomys glareolus and Apodemus agrarius , were found positive for hantaviral antigen in 13.7 % and 4.5 % of the investigated rodents , respectively .
	manualset3
195833	4	415949	7	NULL	NULL	0	NULL	hantaviral antigen 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two species , Clethrionomys glareolus and Apodemus agrarius , were found positive for hantaviral antigen in 13.7 % and 4.5 % of the investigated rodents , respectively .
	manualset3
195834	5	415949	7	NULL	NULL	0	NULL	 13.7 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two species , Clethrionomys glareolus and Apodemus agrarius , were found positive for hantaviral antigen in 13.7 % and 4.5 % of the investigated rodents , respectively .
	manualset3
195835	6	415949	7	NULL	NULL	0	NULL	4.5 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two species , Clethrionomys glareolus and Apodemus agrarius , were found positive for hantaviral antigen in 13.7 % and 4.5 % of the investigated rodents , respectively .
	manualset3
195836	7	415949	7	NULL	NULL	0	NULL	investigated rodents	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two species , Clethrionomys glareolus and Apodemus agrarius , were found positive for hantaviral antigen in 13.7 % and 4.5 % of the investigated rodents , respectively .
	manualset3
195837	1	415950	7	NULL	NULL	0	NULL	Two strain combinations	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two strain combinations with major histocompatibility complex class I and class II and minor histocompatibility complex disparity had 20 % and 33 % survival of more than 100 days , but the other 11 combinations , including four that were fully allogeneic and all with only class I , class II or minor disparities , yielded 45 % to 100 % survival of more than 100 days .
	manualset3
195838	2	415950	7	NULL	NULL	0	NULL	major histocompatibility complex class I	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two strain combinations with major histocompatibility complex class I and class II and minor histocompatibility complex disparity had 20 % and 33 % survival of more than 100 days , but the other 11 combinations , including four that were fully allogeneic and all with only class I , class II or minor disparities , yielded 45 % to 100 % survival of more than 100 days .
	manualset3
195839	3	415950	7	NULL	NULL	0	NULL	major histocompatibility complex class II	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two strain combinations with major histocompatibility complex class I and class II and minor histocompatibility complex disparity had 20 % and 33 % survival of more than 100 days , but the other 11 combinations , including four that were fully allogeneic and all with only class I , class II or minor disparities , yielded 45 % to 100 % survival of more than 100 days .
	manualset3
195840	4	415950	7	NULL	NULL	0	NULL	minor histocompatibility complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two strain combinations with major histocompatibility complex class I and class II and minor histocompatibility complex disparity had 20 % and 33 % survival of more than 100 days , but the other 11 combinations , including four that were fully allogeneic and all with only class I , class II or minor disparities , yielded 45 % to 100 % survival of more than 100 days .
	manualset3
195841	5	415950	7	NULL	NULL	0	NULL	20 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two strain combinations with major histocompatibility complex class I and class II and minor histocompatibility complex disparity had 20 % and 33 % survival of more than 100 days , but the other 11 combinations , including four that were fully allogeneic and all with only class I , class II or minor disparities , yielded 45 % to 100 % survival of more than 100 days .
	manualset3
195842	6	415950	7	NULL	NULL	0	NULL	33 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two strain combinations with major histocompatibility complex class I and class II and minor histocompatibility complex disparity had 20 % and 33 % survival of more than 100 days , but the other 11 combinations , including four that were fully allogeneic and all with only class I , class II or minor disparities , yielded 45 % to 100 % survival of more than 100 days .
	manualset3
195843	7	415950	7	NULL	NULL	0	NULL	survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two strain combinations with major histocompatibility complex class I and class II and minor histocompatibility complex disparity had 20 % and 33 % survival of more than 100 days , but the other 11 combinations , including four that were fully allogeneic and all with only class I , class II or minor disparities , yielded 45 % to 100 % survival of more than 100 days .
	manualset3
195844	8	415950	7	NULL	NULL	0	NULL	100 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Two strain combinations with major histocompatibility complex class I and class II and minor histocompatibility complex disparity had 20 % and 33 % survival of more than 100 days , but the other 11 combinations , including four that were fully allogeneic and all with only class I , class II or minor disparities , yielded 45 % to 100 % survival of more than 100 days .
	manualset3
195845	9	415950	7	NULL	NULL	0	NULL	11 combinations	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two strain combinations with major histocompatibility complex class I and class II and minor histocompatibility complex disparity had 20 % and 33 % survival of more than 100 days , but the other 11 combinations , including four that were fully allogeneic and all with only class I , class II or minor disparities , yielded 45 % to 100 % survival of more than 100 days .
	manualset3
195846	10	415950	7	NULL	NULL	0	NULL	four 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two strain combinations with major histocompatibility complex class I and class II and minor histocompatibility complex disparity had 20 % and 33 % survival of more than 100 days , but the other 11 combinations , including four that were fully allogeneic and all with only class I , class II or minor disparities , yielded 45 % to 100 % survival of more than 100 days .
	manualset3
195847	11	415950	7	NULL	NULL	0	NULL	fully allogeneic	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two strain combinations with major histocompatibility complex class I and class II and minor histocompatibility complex disparity had 20 % and 33 % survival of more than 100 days , but the other 11 combinations , including four that were fully allogeneic and all with only class I , class II or minor disparities , yielded 45 % to 100 % survival of more than 100 days .
	manualset3
195848	12	415950	7	NULL	NULL	0	NULL	class I	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two strain combinations with major histocompatibility complex class I and class II and minor histocompatibility complex disparity had 20 % and 33 % survival of more than 100 days , but the other 11 combinations , including four that were fully allogeneic and all with only class I , class II or minor disparities , yielded 45 % to 100 % survival of more than 100 days .
	manualset3
195849	13	415950	7	NULL	NULL	0	NULL	class II	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two strain combinations with major histocompatibility complex class I and class II and minor histocompatibility complex disparity had 20 % and 33 % survival of more than 100 days , but the other 11 combinations , including four that were fully allogeneic and all with only class I , class II or minor disparities , yielded 45 % to 100 % survival of more than 100 days .
	manualset3
195850	14	415950	7	NULL	NULL	0	NULL	minor disparities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two strain combinations with major histocompatibility complex class I and class II and minor histocompatibility complex disparity had 20 % and 33 % survival of more than 100 days , but the other 11 combinations , including four that were fully allogeneic and all with only class I , class II or minor disparities , yielded 45 % to 100 % survival of more than 100 days .
	manualset3
195851	15	415950	7	NULL	NULL	0	NULL	45 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two strain combinations with major histocompatibility complex class I and class II and minor histocompatibility complex disparity had 20 % and 33 % survival of more than 100 days , but the other 11 combinations , including four that were fully allogeneic and all with only class I , class II or minor disparities , yielded 45 % to 100 % survival of more than 100 days .
	manualset3
195852	16	415950	7	NULL	NULL	0	NULL	100 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two strain combinations with major histocompatibility complex class I and class II and minor histocompatibility complex disparity had 20 % and 33 % survival of more than 100 days , but the other 11 combinations , including four that were fully allogeneic and all with only class I , class II or minor disparities , yielded 45 % to 100 % survival of more than 100 days .
	manualset3
195853	17	415950	7	NULL	NULL	0	NULL	survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two strain combinations with major histocompatibility complex class I and class II and minor histocompatibility complex disparity had 20 % and 33 % survival of more than 100 days , but the other 11 combinations , including four that were fully allogeneic and all with only class I , class II or minor disparities , yielded 45 % to 100 % survival of more than 100 days .
	manualset3
195854	18	415950	7	NULL	NULL	0	NULL	100 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Two strain combinations with major histocompatibility complex class I and class II and minor histocompatibility complex disparity had 20 % and 33 % survival of more than 100 days , but the other 11 combinations , including four that were fully allogeneic and all with only class I , class II or minor disparities , yielded 45 % to 100 % survival of more than 100 days .
	manualset3
195855	1	415951	7	NULL	NULL	0	NULL	Two strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two strains of E. coli were inhibited by 25 micrograms/ml .
	manualset3
195857	2	415951	7	NULL	NULL	0	NULL	E. coli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two strains of E. coli were inhibited by 25 micrograms/ml .
	manualset3
195858	3	415951	7	NULL	NULL	0	NULL	25 micrograms/ml 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two strains of E. coli were inhibited by 25 micrograms/ml .
	manualset3
195859	1	415952	7	NULL	NULL	0	NULL	Two tentative ideas	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two tentative ideas , making recycle use of iron and the application of acid waste water in the process , were proposed .
	manualset3
195860	2	415952	7	NULL	NULL	0	NULL	recycle use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two tentative ideas , making recycle use of iron and the application of acid waste water in the process , were proposed .
	manualset3
195861	3	415952	7	NULL	NULL	0	NULL	 iron	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two tentative ideas , making recycle use of iron and the application of acid waste water in the process , were proposed .
	manualset3
195862	4	415952	7	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two tentative ideas , making recycle use of iron and the application of acid waste water in the process , were proposed .
	manualset3
195863	5	415952	7	NULL	NULL	0	NULL	acid waste water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two tentative ideas , making recycle use of iron and the application of acid waste water in the process , were proposed .
	manualset3
195864	6	415952	7	NULL	NULL	0	NULL	process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two tentative ideas , making recycle use of iron and the application of acid waste water in the process , were proposed .
	manualset3
195865	1	415953	7	NULL	NULL	0	NULL	Two transformed P. pastoris clones	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two transformed P. pastoris clones containing the multicopy of mRAL and ProRAL genes were separately selected for the production of recombinant enzymes .
	manualset3
195866	2	415953	7	NULL	NULL	0	NULL	multicopy	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Two transformed P. pastoris clones containing the multicopy of mRAL and ProRAL genes were separately selected for the production of recombinant enzymes .
	manualset3
195867	3	415953	7	NULL	NULL	0	NULL	mRAL genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Two transformed P. pastoris clones containing the multicopy of mRAL and ProRAL genes were separately selected for the production of recombinant enzymes .
	manualset3
195868	4	415953	7	NULL	NULL	0	NULL	ProRAL gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Two transformed P. pastoris clones containing the multicopy of mRAL and ProRAL genes were separately selected for the production of recombinant enzymes .
	manualset3
195869	5	415953	7	NULL	NULL	0	NULL	production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two transformed P. pastoris clones containing the multicopy of mRAL and ProRAL genes were separately selected for the production of recombinant enzymes .
	manualset3
195870	6	415953	7	NULL	NULL	NULL	NULL	recombinant enzymes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two transformed P. pastoris clones containing the multicopy of mRAL and ProRAL genes were separately selected for the production of recombinant enzymes .
	manualset3
195871	1	415954	7	NULL	NULL	0	NULL	Two types 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two types of ligament injuries common in skiing are the isolated ruptures of the anterior cruciate and ruptures of the medial collateral , either with or without rupture of the anterior cruciate .
	manualset3
195872	2	415954	7	NULL	NULL	0	NULL	ligament injuries	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two types of ligament injuries common in skiing are the isolated ruptures of the anterior cruciate and ruptures of the medial collateral , either with or without rupture of the anterior cruciate .
	manualset3
195873	3	415954	7	NULL	NULL	0	NULL	skiing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two types of ligament injuries common in skiing are the isolated ruptures of the anterior cruciate and ruptures of the medial collateral , either with or without rupture of the anterior cruciate .
	manualset3
195874	4	415954	7	NULL	NULL	0	NULL	isolated ruptures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two types of ligament injuries common in skiing are the isolated ruptures of the anterior cruciate and ruptures of the medial collateral , either with or without rupture of the anterior cruciate .
	manualset3
195875	5	415954	7	NULL	NULL	0	NULL	anterior cruciate	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Two types of ligament injuries common in skiing are the isolated ruptures of the anterior cruciate and ruptures of the medial collateral , either with or without rupture of the anterior cruciate .
	manualset3
195876	6	415954	7	NULL	NULL	0	NULL	ruptures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two types of ligament injuries common in skiing are the isolated ruptures of the anterior cruciate and ruptures of the medial collateral , either with or without rupture of the anterior cruciate .
	manualset3
195877	7	415954	7	NULL	NULL	0	NULL	medial collateral	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Two types of ligament injuries common in skiing are the isolated ruptures of the anterior cruciate and ruptures of the medial collateral , either with or without rupture of the anterior cruciate .
	manualset3
195878	8	415954	7	NULL	NULL	0	NULL	 rupture	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two types of ligament injuries common in skiing are the isolated ruptures of the anterior cruciate and ruptures of the medial collateral , either with or without rupture of the anterior cruciate .
	manualset3
195879	9	415954	7	NULL	NULL	0	NULL	 anterior cruciate	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Two types of ligament injuries common in skiing are the isolated ruptures of the anterior cruciate and ruptures of the medial collateral , either with or without rupture of the anterior cruciate .
	manualset3
195880	1	415955	7	NULL	NULL	0	NULL	Two unique psychrophilic strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two unique psychrophilic strains ( CMS 76rT and CMS 81yT ) were isolated from a cyanobacterial mat sample from a pond in Wright Valley , McMurdo , Antarctica .
	manualset3
195881	2	415955	7	NULL	NULL	0	NULL	CMS 76rT	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two unique psychrophilic strains ( CMS 76rT and CMS 81yT ) were isolated from a cyanobacterial mat sample from a pond in Wright Valley , McMurdo , Antarctica .
	manualset3
195882	3	415955	7	NULL	NULL	0	NULL	CMS 81yT	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two unique psychrophilic strains ( CMS 76rT and CMS 81yT ) were isolated from a cyanobacterial mat sample from a pond in Wright Valley , McMurdo , Antarctica .
	manualset3
195883	4	415955	7	NULL	NULL	0	NULL	cyanobacterial mat sample	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two unique psychrophilic strains ( CMS 76rT and CMS 81yT ) were isolated from a cyanobacterial mat sample from a pond in Wright Valley , McMurdo , Antarctica .
	manualset3
195884	5	415955	7	NULL	NULL	0	NULL	 pond	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Two unique psychrophilic strains ( CMS 76rT and CMS 81yT ) were isolated from a cyanobacterial mat sample from a pond in Wright Valley , McMurdo , Antarctica .
	manualset3
195885	6	415955	7	NULL	NULL	0	NULL	Wright Valley	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Two unique psychrophilic strains ( CMS 76rT and CMS 81yT ) were isolated from a cyanobacterial mat sample from a pond in Wright Valley , McMurdo , Antarctica .
	manualset3
195886	7	415955	7	NULL	NULL	0	NULL	McMurdo	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Two unique psychrophilic strains ( CMS 76rT and CMS 81yT ) were isolated from a cyanobacterial mat sample from a pond in Wright Valley , McMurdo , Antarctica .
	manualset3
195887	8	415955	7	NULL	NULL	0	NULL	Antarctica	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Two unique psychrophilic strains ( CMS 76rT and CMS 81yT ) were isolated from a cyanobacterial mat sample from a pond in Wright Valley , McMurdo , Antarctica .
	manualset3
195888	1	415956	7	NULL	NULL	0	NULL	Two unusual cases	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two unusual cases of canine prostatitis : prostatitis in a castrated dog and preputial oedema in an intact male .
	manualset3
195889	2	415956	7	NULL	NULL	0	NULL	canine prostatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two unusual cases of canine prostatitis : prostatitis in a castrated dog and preputial oedema in an intact male .
	manualset3
195890	3	415956	7	NULL	NULL	0	NULL	prostatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two unusual cases of canine prostatitis : prostatitis in a castrated dog and preputial oedema in an intact male .
	manualset3
195891	4	415956	7	NULL	NULL	0	NULL	 castrated dog	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two unusual cases of canine prostatitis : prostatitis in a castrated dog and preputial oedema in an intact male .
	manualset3
195892	5	415956	7	NULL	NULL	0	NULL	preputial oedema	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two unusual cases of canine prostatitis : prostatitis in a castrated dog and preputial oedema in an intact male .
	manualset3
195893	6	415956	7	NULL	NULL	0	NULL	male	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Two unusual cases of canine prostatitis : prostatitis in a castrated dog and preputial oedema in an intact male .
	manualset3
195894	1	415957	7	NULL	NULL	0	NULL	Two viral proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two viral proteins , E1B-55 kDa and E4orf6 , are both necessary for these effects .
	manualset3
195895	2	415957	7	NULL	NULL	0	NULL	E1B-55 kDa	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Two viral proteins , E1B-55 kDa and E4orf6 , are both necessary for these effects .
	manualset3
195896	3	415957	7	NULL	NULL	0	NULL	E4orf6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Two viral proteins , E1B-55 kDa and E4orf6 , are both necessary for these effects .
	manualset3
195897	4	415957	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two viral proteins , E1B-55 kDa and E4orf6 , are both necessary for these effects .
	manualset3
195898	1	415958	7	NULL	NULL	0	NULL	Two weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Two weeks after nerve crush , the hind legs of three groups of rats were immobilized with bilateral casts at the knee and ankle joints and the fourth group was a control group .
	manualset3
195899	2	415958	7	NULL	NULL	0	NULL	nerve crush	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two weeks after nerve crush , the hind legs of three groups of rats were immobilized with bilateral casts at the knee and ankle joints and the fourth group was a control group .
	manualset3
195900	3	415958	7	NULL	NULL	0	NULL	hind legs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Two weeks after nerve crush , the hind legs of three groups of rats were immobilized with bilateral casts at the knee and ankle joints and the fourth group was a control group .
	manualset3
195901	4	415958	7	NULL	NULL	0	NULL	 three groups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two weeks after nerve crush , the hind legs of three groups of rats were immobilized with bilateral casts at the knee and ankle joints and the fourth group was a control group .
	manualset3
195902	5	415958	7	NULL	NULL	0	NULL	 rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two weeks after nerve crush , the hind legs of three groups of rats were immobilized with bilateral casts at the knee and ankle joints and the fourth group was a control group .
	manualset3
195903	6	415958	7	NULL	NULL	0	NULL	bilateral casts	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Two weeks after nerve crush , the hind legs of three groups of rats were immobilized with bilateral casts at the knee and ankle joints and the fourth group was a control group .
	manualset3
195904	7	415958	7	NULL	NULL	0	NULL	 knee joint	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Two weeks after nerve crush , the hind legs of three groups of rats were immobilized with bilateral casts at the knee and ankle joints and the fourth group was a control group .
	manualset3
195905	8	415958	7	NULL	NULL	0	NULL	ankle joints	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Two weeks after nerve crush , the hind legs of three groups of rats were immobilized with bilateral casts at the knee and ankle joints and the fourth group was a control group .
	manualset3
195906	9	415958	7	NULL	NULL	0	NULL	fourth group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two weeks after nerve crush , the hind legs of three groups of rats were immobilized with bilateral casts at the knee and ankle joints and the fourth group was a control group .
	manualset3
195907	10	415958	7	NULL	NULL	0	NULL	control group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two weeks after nerve crush , the hind legs of three groups of rats were immobilized with bilateral casts at the knee and ankle joints and the fourth group was a control group .
	manualset3
195908	1	415959	7	NULL	NULL	NULL	NULL	Two whole genome scans	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two whole genome scans from Japan and from the US identified a locus on chromosome 8q24 that showed evidence for linkage with AITD and HT .
	manualset3
195909	2	415959	7	NULL	NULL	0	NULL	Japan	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Two whole genome scans from Japan and from the US identified a locus on chromosome 8q24 that showed evidence for linkage with AITD and HT .
	manualset3
195910	3	415959	7	NULL	NULL	0	NULL	 US 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Two whole genome scans from Japan and from the US identified a locus on chromosome 8q24 that showed evidence for linkage with AITD and HT .
	manualset3
195911	4	415959	7	NULL	NULL	0	NULL	locus	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Two whole genome scans from Japan and from the US identified a locus on chromosome 8q24 that showed evidence for linkage with AITD and HT .
	manualset3
195912	5	415959	7	NULL	NULL	0	NULL	chromosome 8q24	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Two whole genome scans from Japan and from the US identified a locus on chromosome 8q24 that showed evidence for linkage with AITD and HT .
	manualset3
195913	6	415959	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two whole genome scans from Japan and from the US identified a locus on chromosome 8q24 that showed evidence for linkage with AITD and HT .
	manualset3
195914	7	415959	7	NULL	NULL	0	NULL	 linkage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two whole genome scans from Japan and from the US identified a locus on chromosome 8q24 that showed evidence for linkage with AITD and HT .
	manualset3
195915	8	415959	7	NULL	NULL	0	NULL	AITD 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two whole genome scans from Japan and from the US identified a locus on chromosome 8q24 that showed evidence for linkage with AITD and HT .
	manualset3
195916	9	415959	7	NULL	NULL	0	NULL	HT	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two whole genome scans from Japan and from the US identified a locus on chromosome 8q24 that showed evidence for linkage with AITD and HT .
	manualset3
195917	1	415960	7	NULL	NULL	0	NULL	several courses	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After several courses of chemotherapy , the patient improved neurologically and could walk independently .
	manualset3
195918	2	415960	7	NULL	NULL	0	NULL	 chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After several courses of chemotherapy , the patient improved neurologically and could walk independently .
	manualset3
195919	3	415960	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	After several courses of chemotherapy , the patient improved neurologically and could walk independently .
	manualset3
195920	1	415961	7	NULL	NULL	0	NULL	Type-2 diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Type-2 diabetes is associated with an excessively high mortality and morbidity due to cardiovascular disease .
	manualset3
195921	2	415961	7	NULL	NULL	0	NULL	high mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Type-2 diabetes is associated with an excessively high mortality and morbidity due to cardiovascular disease .
	manualset3
195922	3	415961	7	NULL	NULL	0	NULL	high morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Type-2 diabetes is associated with an excessively high mortality and morbidity due to cardiovascular disease .
	manualset3
195923	4	415961	7	NULL	NULL	0	NULL	cardiovascular disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Type-2 diabetes is associated with an excessively high mortality and morbidity due to cardiovascular disease .
	manualset3
195924	1	415962	7	NULL	NULL	0	NULL	Type 2 diabetes 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Type 2 diabetes , glucose homeostasis and incident atrial fibrillation : the Atherosclerosis Risk in Communities study .
	manualset3
195925	2	415962	7	NULL	NULL	0	NULL	glucose homeostasis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Type 2 diabetes , glucose homeostasis and incident atrial fibrillation : the Atherosclerosis Risk in Communities study .
	manualset3
195926	3	415962	7	NULL	NULL	NULL	NULL	incident atrial fibrillation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Type 2 diabetes , glucose homeostasis and incident atrial fibrillation : the Atherosclerosis Risk in Communities study .
	manualset3
195927	4	415962	7	NULL	NULL	0	NULL	Atherosclerosis Risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Type 2 diabetes , glucose homeostasis and incident atrial fibrillation : the Atherosclerosis Risk in Communities study .
	manualset3
195928	5	415962	7	NULL	NULL	0	NULL	Communities study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Type 2 diabetes , glucose homeostasis and incident atrial fibrillation : the Atherosclerosis Risk in Communities study .
	manualset3
195929	1	415963	7	NULL	NULL	0	NULL	Type 2 diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Type 2 diabetes is likely to be a polygenic disease , with a combination of major and minor genes affecting obesity , insulin secretion , and insulin action .
	manualset3
195930	2	415963	7	NULL	NULL	0	NULL	polygenic disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Type 2 diabetes is likely to be a polygenic disease , with a combination of major and minor genes affecting obesity , insulin secretion , and insulin action .
	manualset3
195931	3	415963	7	NULL	NULL	0	NULL	 combination	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Type 2 diabetes is likely to be a polygenic disease , with a combination of major and minor genes affecting obesity , insulin secretion , and insulin action .
	manualset3
195932	4	415963	7	NULL	NULL	0	NULL	major genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Type 2 diabetes is likely to be a polygenic disease , with a combination of major and minor genes affecting obesity , insulin secretion , and insulin action .
	manualset3
195933	5	415963	7	NULL	NULL	0	NULL	minor genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Type 2 diabetes is likely to be a polygenic disease , with a combination of major and minor genes affecting obesity , insulin secretion , and insulin action .
	manualset3
195934	6	415963	7	NULL	NULL	0	NULL	obesity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Type 2 diabetes is likely to be a polygenic disease , with a combination of major and minor genes affecting obesity , insulin secretion , and insulin action .
	manualset3
195935	7	415963	7	NULL	NULL	0	NULL	insulin secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Type 2 diabetes is likely to be a polygenic disease , with a combination of major and minor genes affecting obesity , insulin secretion , and insulin action .
	manualset3
195936	8	415963	7	NULL	NULL	0	NULL	insulin action 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Type 2 diabetes is likely to be a polygenic disease , with a combination of major and minor genes affecting obesity , insulin secretion , and insulin action .
	manualset3
195937	1	415964	7	NULL	NULL	0	NULL	Type 2 diabetes mellitus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Type 2 diabetes mellitus is the consequence of both insulin resistance and impaired insulin secretion .
	manualset3
195938	2	415964	7	NULL	NULL	0	NULL	insulin resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Type 2 diabetes mellitus is the consequence of both insulin resistance and impaired insulin secretion .
	manualset3
195939	3	415964	7	NULL	NULL	NULL	NULL	impaired insulin secretion	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Type 2 diabetes mellitus is the consequence of both insulin resistance and impaired insulin secretion .
	manualset3
195940	1	415965	7	NULL	NULL	0	NULL	Type 2 first branchial cleft cyst	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Type 2 first branchial cleft cyst presenting as childhood deafness .
	manualset3
195941	2	415965	7	NULL	NULL	0	NULL	childhood deafness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Type 2 first branchial cleft cyst presenting as childhood deafness .
	manualset3
195942	1	415966	7	NULL	NULL	0	NULL	Type I R genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Type I R genes tend to reduce the microsynteny of their flanking regions significantly more than type II R genes , and their flanking regions have slightly but significantly lower G/C content than those of type II R genes .
	manualset3
195943	2	415966	7	NULL	NULL	0	NULL	microsynteny	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Type I R genes tend to reduce the microsynteny of their flanking regions significantly more than type II R genes , and their flanking regions have slightly but significantly lower G/C content than those of type II R genes .
	manualset3
195944	3	415966	7	NULL	NULL	0	NULL	 flanking regions	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Type I R genes tend to reduce the microsynteny of their flanking regions significantly more than type II R genes , and their flanking regions have slightly but significantly lower G/C content than those of type II R genes .
	manualset3
195945	4	415966	7	NULL	NULL	0	NULL	type II R genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Type I R genes tend to reduce the microsynteny of their flanking regions significantly more than type II R genes , and their flanking regions have slightly but significantly lower G/C content than those of type II R genes .
	manualset3
195946	5	415966	7	NULL	NULL	0	NULL	flanking regions	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Type I R genes tend to reduce the microsynteny of their flanking regions significantly more than type II R genes , and their flanking regions have slightly but significantly lower G/C content than those of type II R genes .
	manualset3
195947	6	415966	7	NULL	NULL	0	NULL	lower G/C content 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Type I R genes tend to reduce the microsynteny of their flanking regions significantly more than type II R genes , and their flanking regions have slightly but significantly lower G/C content than those of type II R genes .
	manualset3
195948	7	415966	7	NULL	NULL	0	NULL	type II R genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Type I R genes tend to reduce the microsynteny of their flanking regions significantly more than type II R genes , and their flanking regions have slightly but significantly lower G/C content than those of type II R genes .
	manualset3
195949	1	415967	7	NULL	NULL	0	NULL	Type I RFLPs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Type I RFLPs are those observed at 4.3 kilobase ( kb ) and 1.9 kb by AvaI digestion for PLC-gamma probe and at 1.9 kb by AccI digestion for PLC-beta probe , where RFLP banding patterns are conserved in two hypertensive ( SHR and SHR-SP ) and one normotensive ( Sprague-Dawley ) strains .
	manualset3
195950	2	415967	7	NULL	NULL	0	NULL	 4.3 kilobase ( kb )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Type I RFLPs are those observed at 4.3 kilobase ( kb ) and 1.9 kb by AvaI digestion for PLC-gamma probe and at 1.9 kb by AccI digestion for PLC-beta probe , where RFLP banding patterns are conserved in two hypertensive ( SHR and SHR-SP ) and one normotensive ( Sprague-Dawley ) strains .
	manualset3
195951	3	415967	7	NULL	NULL	0	NULL	1.9 kb	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Type I RFLPs are those observed at 4.3 kilobase ( kb ) and 1.9 kb by AvaI digestion for PLC-gamma probe and at 1.9 kb by AccI digestion for PLC-beta probe , where RFLP banding patterns are conserved in two hypertensive ( SHR and SHR-SP ) and one normotensive ( Sprague-Dawley ) strains .
	manualset3
195952	4	415967	7	NULL	NULL	0	NULL	AvaI digestion	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Type I RFLPs are those observed at 4.3 kilobase ( kb ) and 1.9 kb by AvaI digestion for PLC-gamma probe and at 1.9 kb by AccI digestion for PLC-beta probe , where RFLP banding patterns are conserved in two hypertensive ( SHR and SHR-SP ) and one normotensive ( Sprague-Dawley ) strains .
	manualset3
195953	5	415967	7	NULL	NULL	NULL	NULL	PLC-gamma probe	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Type I RFLPs are those observed at 4.3 kilobase ( kb ) and 1.9 kb by AvaI digestion for PLC-gamma probe and at 1.9 kb by AccI digestion for PLC-beta probe , where RFLP banding patterns are conserved in two hypertensive ( SHR and SHR-SP ) and one normotensive ( Sprague-Dawley ) strains .
	manualset3
195954	6	415967	7	NULL	NULL	0	NULL	1.9 kb	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Type I RFLPs are those observed at 4.3 kilobase ( kb ) and 1.9 kb by AvaI digestion for PLC-gamma probe and at 1.9 kb by AccI digestion for PLC-beta probe , where RFLP banding patterns are conserved in two hypertensive ( SHR and SHR-SP ) and one normotensive ( Sprague-Dawley ) strains .
	manualset3
195955	7	415967	7	NULL	NULL	0	NULL	AccI digestion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Type I RFLPs are those observed at 4.3 kilobase ( kb ) and 1.9 kb by AvaI digestion for PLC-gamma probe and at 1.9 kb by AccI digestion for PLC-beta probe , where RFLP banding patterns are conserved in two hypertensive ( SHR and SHR-SP ) and one normotensive ( Sprague-Dawley ) strains .
	manualset3
195956	8	415967	7	NULL	NULL	0	NULL	PLC-beta probe	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Type I RFLPs are those observed at 4.3 kilobase ( kb ) and 1.9 kb by AvaI digestion for PLC-gamma probe and at 1.9 kb by AccI digestion for PLC-beta probe , where RFLP banding patterns are conserved in two hypertensive ( SHR and SHR-SP ) and one normotensive ( Sprague-Dawley ) strains .
	manualset3
195957	9	415967	7	NULL	NULL	0	NULL	RFLP banding patterns	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Type I RFLPs are those observed at 4.3 kilobase ( kb ) and 1.9 kb by AvaI digestion for PLC-gamma probe and at 1.9 kb by AccI digestion for PLC-beta probe , where RFLP banding patterns are conserved in two hypertensive ( SHR and SHR-SP ) and one normotensive ( Sprague-Dawley ) strains .
	manualset3
195958	10	415967	7	NULL	NULL	0	NULL	two hypertensive strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Type I RFLPs are those observed at 4.3 kilobase ( kb ) and 1.9 kb by AvaI digestion for PLC-gamma probe and at 1.9 kb by AccI digestion for PLC-beta probe , where RFLP banding patterns are conserved in two hypertensive ( SHR and SHR-SP ) and one normotensive ( Sprague-Dawley ) strains .
	manualset3
195959	11	415967	7	NULL	NULL	0	NULL	SHR	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Type I RFLPs are those observed at 4.3 kilobase ( kb ) and 1.9 kb by AvaI digestion for PLC-gamma probe and at 1.9 kb by AccI digestion for PLC-beta probe , where RFLP banding patterns are conserved in two hypertensive ( SHR and SHR-SP ) and one normotensive ( Sprague-Dawley ) strains .
	manualset3
195960	12	415967	7	NULL	NULL	0	NULL	SHR-SP	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Type I RFLPs are those observed at 4.3 kilobase ( kb ) and 1.9 kb by AvaI digestion for PLC-gamma probe and at 1.9 kb by AccI digestion for PLC-beta probe , where RFLP banding patterns are conserved in two hypertensive ( SHR and SHR-SP ) and one normotensive ( Sprague-Dawley ) strains .
	manualset3
195961	13	415967	7	NULL	NULL	0	NULL	one normotensive strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Type I RFLPs are those observed at 4.3 kilobase ( kb ) and 1.9 kb by AvaI digestion for PLC-gamma probe and at 1.9 kb by AccI digestion for PLC-beta probe , where RFLP banding patterns are conserved in two hypertensive ( SHR and SHR-SP ) and one normotensive ( Sprague-Dawley ) strains .
	manualset3
195962	14	415967	7	NULL	NULL	0	NULL	Sprague-Dawley strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Type I RFLPs are those observed at 4.3 kilobase ( kb ) and 1.9 kb by AvaI digestion for PLC-gamma probe and at 1.9 kb by AccI digestion for PLC-beta probe , where RFLP banding patterns are conserved in two hypertensive ( SHR and SHR-SP ) and one normotensive ( Sprague-Dawley ) strains .
	manualset3
195963	1	415968	7	NULL	NULL	0	NULL	Type I cotton MYB transcripts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Type I cotton MYB ( GhMYB-1 , -2 , and -3 ) transcripts were found in all tissue-types examined and were relatively more abundant than those derived from type II GhMYB genes ( GhMYB-4 , -5 , and -6 ) , which showed distinct , tissue-specific expression patterns .
	manualset3
195964	2	415968	7	NULL	NULL	0	NULL	GhMYB-1 transcripts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Type I cotton MYB ( GhMYB-1 , -2 , and -3 ) transcripts were found in all tissue-types examined and were relatively more abundant than those derived from type II GhMYB genes ( GhMYB-4 , -5 , and -6 ) , which showed distinct , tissue-specific expression patterns .
	manualset3
195965	3	415968	7	NULL	NULL	NULL	NULL	GhMYB-2 transcripts	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Type I cotton MYB ( GhMYB-1 , -2 , and -3 ) transcripts were found in all tissue-types examined and were relatively more abundant than those derived from type II GhMYB genes ( GhMYB-4 , -5 , and -6 ) , which showed distinct , tissue-specific expression patterns .
	manualset3
195966	4	415968	7	NULL	NULL	NULL	NULL	GhMYB-3 transcripts	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Type I cotton MYB ( GhMYB-1 , -2 , and -3 ) transcripts were found in all tissue-types examined and were relatively more abundant than those derived from type II GhMYB genes ( GhMYB-4 , -5 , and -6 ) , which showed distinct , tissue-specific expression patterns .
	manualset3
195967	5	415968	7	NULL	NULL	0	NULL	 tissue-types	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Type I cotton MYB ( GhMYB-1 , -2 , and -3 ) transcripts were found in all tissue-types examined and were relatively more abundant than those derived from type II GhMYB genes ( GhMYB-4 , -5 , and -6 ) , which showed distinct , tissue-specific expression patterns .
	manualset3
195968	6	415968	7	NULL	NULL	0	NULL	type II GhMYB genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Type I cotton MYB ( GhMYB-1 , -2 , and -3 ) transcripts were found in all tissue-types examined and were relatively more abundant than those derived from type II GhMYB genes ( GhMYB-4 , -5 , and -6 ) , which showed distinct , tissue-specific expression patterns .
	manualset3
195969	7	415968	7	NULL	NULL	0	NULL	GhMYB-4 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Type I cotton MYB ( GhMYB-1 , -2 , and -3 ) transcripts were found in all tissue-types examined and were relatively more abundant than those derived from type II GhMYB genes ( GhMYB-4 , -5 , and -6 ) , which showed distinct , tissue-specific expression patterns .
	manualset3
195970	8	415968	7	NULL	NULL	0	NULL	GhMYB-5 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Type I cotton MYB ( GhMYB-1 , -2 , and -3 ) transcripts were found in all tissue-types examined and were relatively more abundant than those derived from type II GhMYB genes ( GhMYB-4 , -5 , and -6 ) , which showed distinct , tissue-specific expression patterns .
	manualset3
195971	9	415968	7	NULL	NULL	0	NULL	GhMYB-6 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Type I cotton MYB ( GhMYB-1 , -2 , and -3 ) transcripts were found in all tissue-types examined and were relatively more abundant than those derived from type II GhMYB genes ( GhMYB-4 , -5 , and -6 ) , which showed distinct , tissue-specific expression patterns .
	manualset3
195972	10	415968	7	NULL	NULL	NULL	NULL	 tissue-specific expression patterns 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Type I cotton MYB ( GhMYB-1 , -2 , and -3 ) transcripts were found in all tissue-types examined and were relatively more abundant than those derived from type II GhMYB genes ( GhMYB-4 , -5 , and -6 ) , which showed distinct , tissue-specific expression patterns .
	manualset3
195973	1	415969	7	NULL	NULL	NULL	NULL	Type II caged vesicles	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Type II caged vesicles were found in clusters at the boutons , adhered to the active zone , and were also present in axons .
	manualset3
195974	2	415969	7	NULL	NULL	0	NULL	clusters at the boutons	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Type II caged vesicles were found in clusters at the boutons , adhered to the active zone , and were also present in axons .
	manualset3
195975	3	415969	7	NULL	NULL	0	NULL	 active zone	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Type II caged vesicles were found in clusters at the boutons , adhered to the active zone , and were also present in axons .
	manualset3
195976	4	415969	7	NULL	NULL	0	NULL	axons	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Type II caged vesicles were found in clusters at the boutons , adhered to the active zone , and were also present in axons .
	manualset3
195977	1	415970	7	NULL	NULL	0	NULL	Type	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Type of dietary fat and insulin resistance .
	manualset3
195978	2	415970	7	NULL	NULL	0	NULL	dietary fat	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Type of dietary fat and insulin resistance .
	manualset3
195979	3	415970	7	NULL	NULL	0	NULL	insulin resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Type of dietary fat and insulin resistance .
	manualset3
195980	1	415971	7	NULL	NULL	0	NULL	 several years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After several years a slight increase in the amount of serum monoclonal immunoglobulin occurred ; shortly thereafter an aggressive form of multiple myeloma was diagnosed .
	manualset3
195981	2	415971	7	NULL	NULL	0	NULL	slight increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After several years a slight increase in the amount of serum monoclonal immunoglobulin occurred ; shortly thereafter an aggressive form of multiple myeloma was diagnosed .
	manualset3
195982	3	415971	7	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After several years a slight increase in the amount of serum monoclonal immunoglobulin occurred ; shortly thereafter an aggressive form of multiple myeloma was diagnosed .
	manualset3
195983	4	415971	7	NULL	NULL	0	NULL	 serum monoclonal immunoglobulin 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	After several years a slight increase in the amount of serum monoclonal immunoglobulin occurred ; shortly thereafter an aggressive form of multiple myeloma was diagnosed .
	manualset3
195984	5	415971	7	NULL	NULL	0	NULL	aggressive form	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	After several years a slight increase in the amount of serum monoclonal immunoglobulin occurred ; shortly thereafter an aggressive form of multiple myeloma was diagnosed .
	manualset3
195985	6	415971	7	NULL	NULL	0	NULL	multiple myeloma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	After several years a slight increase in the amount of serum monoclonal immunoglobulin occurred ; shortly thereafter an aggressive form of multiple myeloma was diagnosed .
	manualset3
195986	1	415972	7	NULL	NULL	0	NULL	Typha latifolia ( cattail )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Typha latifolia ( cattail ) sequesters arsenic within predominantlyferric iron root coatings , thus decreasing mobility of this toxic element in wetland sediments .
	manualset3
195987	2	415972	7	NULL	NULL	0	NULL	 arsenic 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Typha latifolia ( cattail ) sequesters arsenic within predominantlyferric iron root coatings , thus decreasing mobility of this toxic element in wetland sediments .
	manualset3
195988	3	415972	7	NULL	NULL	0	NULL	ferric iron root coatings	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Typha latifolia ( cattail ) sequesters arsenic within predominantlyferric iron root coatings , thus decreasing mobility of this toxic element in wetland sediments .
	manualset3
195989	4	415972	7	NULL	NULL	0	NULL	 mobility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Typha latifolia ( cattail ) sequesters arsenic within predominantlyferric iron root coatings , thus decreasing mobility of this toxic element in wetland sediments .
	manualset3
195990	5	415972	7	NULL	NULL	0	NULL	 toxic element 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Typha latifolia ( cattail ) sequesters arsenic within predominantlyferric iron root coatings , thus decreasing mobility of this toxic element in wetland sediments .
	manualset3
195991	6	415972	7	NULL	NULL	0	NULL	 wetland sediments	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Typha latifolia ( cattail ) sequesters arsenic within predominantlyferric iron root coatings , thus decreasing mobility of this toxic element in wetland sediments .
	manualset3
195992	1	415973	7	NULL	NULL	0	NULL	Typical signet-ring cell carcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Typical signet-ring cell carcinomas showed the lowest positivity rate compared with the other histological types of gastric carcinomas .
	manualset3
195993	2	415973	7	NULL	NULL	0	NULL	lowest positivity rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Typical signet-ring cell carcinomas showed the lowest positivity rate compared with the other histological types of gastric carcinomas .
	manualset3
195994	3	415973	7	NULL	NULL	0	NULL	histological types	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Typical signet-ring cell carcinomas showed the lowest positivity rate compared with the other histological types of gastric carcinomas .
	manualset3
195995	4	415973	7	NULL	NULL	0	NULL	gastric carcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Typical signet-ring cell carcinomas showed the lowest positivity rate compared with the other histological types of gastric carcinomas .
	manualset3
195996	1	415974	7	NULL	NULL	0	NULL	 nonadditivity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Typically , nonadditivity ( or `` thermodynamic coupling '' ) is measured from global transitions in concert with a single probe .
	manualset3
195997	2	415974	7	NULL	NULL	0	NULL	thermodynamic coupling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Typically , nonadditivity ( or `` thermodynamic coupling '' ) is measured from global transitions in concert with a single probe .
	manualset3
195998	3	415974	7	NULL	NULL	0	NULL	global transitions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Typically , nonadditivity ( or `` thermodynamic coupling '' ) is measured from global transitions in concert with a single probe .
	manualset3
195999	4	415974	7	NULL	NULL	0	NULL	single probe	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Typically , nonadditivity ( or `` thermodynamic coupling '' ) is measured from global transitions in concert with a single probe .
	manualset3
196000	1	415975	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Typically , patients present with signs and symptoms similar to acute appendicitis ; however , due to prior surgery , the diagnosis is difficult and the rate of appendiceal stump perforation is extremely high .
	manualset3
196001	2	415975	7	NULL	NULL	0	NULL	signs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Typically , patients present with signs and symptoms similar to acute appendicitis ; however , due to prior surgery , the diagnosis is difficult and the rate of appendiceal stump perforation is extremely high .
	manualset3
196002	3	415975	7	NULL	NULL	0	NULL	symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Typically , patients present with signs and symptoms similar to acute appendicitis ; however , due to prior surgery , the diagnosis is difficult and the rate of appendiceal stump perforation is extremely high .
	manualset3
196003	4	415975	7	NULL	NULL	0	NULL	acute appendicitis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Typically , patients present with signs and symptoms similar to acute appendicitis ; however , due to prior surgery , the diagnosis is difficult and the rate of appendiceal stump perforation is extremely high .
	manualset3
196004	5	415975	7	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Typically , patients present with signs and symptoms similar to acute appendicitis ; however , due to prior surgery , the diagnosis is difficult and the rate of appendiceal stump perforation is extremely high .
	manualset3
196005	6	415975	7	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Typically , patients present with signs and symptoms similar to acute appendicitis ; however , due to prior surgery , the diagnosis is difficult and the rate of appendiceal stump perforation is extremely high .
	manualset3
196006	7	415975	7	NULL	NULL	0	NULL	 rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Typically , patients present with signs and symptoms similar to acute appendicitis ; however , due to prior surgery , the diagnosis is difficult and the rate of appendiceal stump perforation is extremely high .
	manualset3
196007	8	415975	7	NULL	NULL	NULL	NULL	appendiceal stump perforation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Typically , patients present with signs and symptoms similar to acute appendicitis ; however , due to prior surgery , the diagnosis is difficult and the rate of appendiceal stump perforation is extremely high .
	manualset3
196008	1	415976	7	NULL	NULL	NULL	NULL	high learning rate	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Typically a high learning rate proves most beneficial as landscape correlation decreases .
	manualset3
196009	2	415976	7	NULL	NULL	0	NULL	 landscape correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Typically a high learning rate proves most beneficial as landscape correlation decreases .
	manualset3
196010	1	415977	7	NULL	NULL	0	NULL	genomics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Typically referred to as genomics , proteomics , and metabonomics or metabolomics , respectively , these methods as independent entities have undoubtedly provided new biological insight that was not attainable a decade ago .
	manualset3
196011	2	415977	7	NULL	NULL	0	NULL	proteomics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Typically referred to as genomics , proteomics , and metabonomics or metabolomics , respectively , these methods as independent entities have undoubtedly provided new biological insight that was not attainable a decade ago .
	manualset3
196012	3	415977	7	NULL	NULL	0	NULL	 metabonomics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Typically referred to as genomics , proteomics , and metabonomics or metabolomics , respectively , these methods as independent entities have undoubtedly provided new biological insight that was not attainable a decade ago .
	manualset3
196013	4	415977	7	NULL	NULL	0	NULL	metabolomics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Typically referred to as genomics , proteomics , and metabonomics or metabolomics , respectively , these methods as independent entities have undoubtedly provided new biological insight that was not attainable a decade ago .
	manualset3
196014	5	415977	7	NULL	NULL	0	NULL	methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Typically referred to as genomics , proteomics , and metabonomics or metabolomics , respectively , these methods as independent entities have undoubtedly provided new biological insight that was not attainable a decade ago .
	manualset3
196015	6	415977	7	NULL	NULL	0	NULL	 independent entities	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Typically referred to as genomics , proteomics , and metabonomics or metabolomics , respectively , these methods as independent entities have undoubtedly provided new biological insight that was not attainable a decade ago .
	manualset3
196016	7	415977	7	NULL	NULL	0	NULL	new biological insight 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Typically referred to as genomics , proteomics , and metabonomics or metabolomics , respectively , these methods as independent entities have undoubtedly provided new biological insight that was not attainable a decade ago .
	manualset3
196017	8	415977	7	NULL	NULL	0	NULL	decade	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Typically referred to as genomics , proteomics , and metabonomics or metabolomics , respectively , these methods as independent entities have undoubtedly provided new biological insight that was not attainable a decade ago .
	manualset3
196018	1	415978	7	NULL	NULL	0	NULL	Tyrosine-phosphorylated Cav1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Tyrosine-phosphorylated Cav1 , therefore , functions as an effector of Rho/ROCK signaling in the regulation of FA turnover and , thereby , tumor cell migration and invasion .
	manualset3
196019	2	415978	7	NULL	NULL	0	NULL	 effector	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Tyrosine-phosphorylated Cav1 , therefore , functions as an effector of Rho/ROCK signaling in the regulation of FA turnover and , thereby , tumor cell migration and invasion .
	manualset3
196020	3	415978	7	NULL	NULL	0	NULL	Rho/ROCK signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Tyrosine-phosphorylated Cav1 , therefore , functions as an effector of Rho/ROCK signaling in the regulation of FA turnover and , thereby , tumor cell migration and invasion .
	manualset3
196021	4	415978	7	NULL	NULL	0	NULL	 regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Tyrosine-phosphorylated Cav1 , therefore , functions as an effector of Rho/ROCK signaling in the regulation of FA turnover and , thereby , tumor cell migration and invasion .
	manualset3
196022	5	415978	7	NULL	NULL	0	NULL	FA turnover	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Tyrosine-phosphorylated Cav1 , therefore , functions as an effector of Rho/ROCK signaling in the regulation of FA turnover and , thereby , tumor cell migration and invasion .
	manualset3
196023	6	415978	7	NULL	NULL	0	NULL	 tumor cell migration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Tyrosine-phosphorylated Cav1 , therefore , functions as an effector of Rho/ROCK signaling in the regulation of FA turnover and , thereby , tumor cell migration and invasion .
	manualset3
196024	7	415978	7	NULL	NULL	0	NULL	 invasion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Tyrosine-phosphorylated Cav1 , therefore , functions as an effector of Rho/ROCK signaling in the regulation of FA turnover and , thereby , tumor cell migration and invasion .
	manualset3
196025	1	415979	7	NULL	NULL	0	NULL	Tyrosine hydroxylase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Tyrosine hydroxylase and Parkinson 's disease .
	manualset3
196026	2	415979	7	NULL	NULL	0	NULL	Parkinson 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Tyrosine hydroxylase and Parkinson 's disease .
	manualset3
196027	1	415980	7	NULL	NULL	0	NULL	Congenital anomalies	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Congenital anomalies in the central nervous system ( 6 ) occult spinal dysraphism ( other than spinal lipoma ) : congenital dermal sinus , tight filum terminale , neurenteric cyst , split cord malformation , and caudal regression syndrome ) .
	manualset3
196028	2	415980	7	NULL	NULL	0	NULL	central nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Congenital anomalies in the central nervous system ( 6 ) occult spinal dysraphism ( other than spinal lipoma ) : congenital dermal sinus , tight filum terminale , neurenteric cyst , split cord malformation , and caudal regression syndrome ) .
	manualset3
196029	3	415980	7	NULL	NULL	0	NULL	occult spinal dysraphism	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Congenital anomalies in the central nervous system ( 6 ) occult spinal dysraphism ( other than spinal lipoma ) : congenital dermal sinus , tight filum terminale , neurenteric cyst , split cord malformation , and caudal regression syndrome ) .
	manualset3
196030	4	415980	7	NULL	NULL	0	NULL	 spinal lipoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Congenital anomalies in the central nervous system ( 6 ) occult spinal dysraphism ( other than spinal lipoma ) : congenital dermal sinus , tight filum terminale , neurenteric cyst , split cord malformation , and caudal regression syndrome ) .
	manualset3
196031	5	415980	7	NULL	NULL	0	NULL	congenital dermal sinus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Congenital anomalies in the central nervous system ( 6 ) occult spinal dysraphism ( other than spinal lipoma ) : congenital dermal sinus , tight filum terminale , neurenteric cyst , split cord malformation , and caudal regression syndrome ) .
	manualset3
196032	6	415980	7	NULL	NULL	0	NULL	tight filum terminale	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Congenital anomalies in the central nervous system ( 6 ) occult spinal dysraphism ( other than spinal lipoma ) : congenital dermal sinus , tight filum terminale , neurenteric cyst , split cord malformation , and caudal regression syndrome ) .
	manualset3
196033	7	415980	7	NULL	NULL	0	NULL	neurenteric cyst	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Congenital anomalies in the central nervous system ( 6 ) occult spinal dysraphism ( other than spinal lipoma ) : congenital dermal sinus , tight filum terminale , neurenteric cyst , split cord malformation , and caudal regression syndrome ) .
	manualset3
196034	8	415980	7	NULL	NULL	0	NULL	split cord malformation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Congenital anomalies in the central nervous system ( 6 ) occult spinal dysraphism ( other than spinal lipoma ) : congenital dermal sinus , tight filum terminale , neurenteric cyst , split cord malformation , and caudal regression syndrome ) .
	manualset3
196035	9	415980	7	NULL	NULL	0	NULL	caudal regression syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Congenital anomalies in the central nervous system ( 6 ) occult spinal dysraphism ( other than spinal lipoma ) : congenital dermal sinus , tight filum terminale , neurenteric cyst , split cord malformation , and caudal regression syndrome ) .
	manualset3
196036	1	415981	7	NULL	NULL	0	NULL	U46619	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	U46619 increased protein kinase C activity in the particulate fraction of vascular smooth muscle cells .
	manualset3
196037	2	415981	7	NULL	NULL	0	NULL	protein kinase C activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	U46619 increased protein kinase C activity in the particulate fraction of vascular smooth muscle cells .
	manualset3
196038	3	415981	7	NULL	NULL	0	NULL	particulate fraction	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	U46619 increased protein kinase C activity in the particulate fraction of vascular smooth muscle cells .
	manualset3
196039	4	415981	7	NULL	NULL	0	NULL	vascular smooth muscle cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	U46619 increased protein kinase C activity in the particulate fraction of vascular smooth muscle cells .
	manualset3
196040	1	415982	7	NULL	NULL	0	NULL	UCP2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	UCP2 is a recently identified fatty acid-responsive mitochondrial inner membrane carrier protein showing wide tissue distribution with a substantially increased presence in fatty liver .
	manualset3
196041	2	415982	7	NULL	NULL	0	NULL	fatty acid-responsive mitochondrial inner membrane carrier protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	UCP2 is a recently identified fatty acid-responsive mitochondrial inner membrane carrier protein showing wide tissue distribution with a substantially increased presence in fatty liver .
	manualset3
196042	3	415982	7	NULL	NULL	0	NULL	 tissue distribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	UCP2 is a recently identified fatty acid-responsive mitochondrial inner membrane carrier protein showing wide tissue distribution with a substantially increased presence in fatty liver .
	manualset3
196043	4	415982	7	NULL	NULL	0	NULL	 fatty liver	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	UCP2 is a recently identified fatty acid-responsive mitochondrial inner membrane carrier protein showing wide tissue distribution with a substantially increased presence in fatty liver .
	manualset3
196044	1	415983	7	NULL	NULL	0	NULL	UCP2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	UCP2 is present in drug-resistant lines of various cancer cells and in human colon cancer .
	manualset3
196045	2	415983	7	NULL	NULL	0	NULL	drug-resistant lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	UCP2 is present in drug-resistant lines of various cancer cells and in human colon cancer .
	manualset3
196046	3	415983	7	NULL	NULL	0	NULL	cancer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	UCP2 is present in drug-resistant lines of various cancer cells and in human colon cancer .
	manualset3
196047	4	415983	7	NULL	NULL	0	NULL	human colon cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	UCP2 is present in drug-resistant lines of various cancer cells and in human colon cancer .
	manualset3
196048	1	415984	7	NULL	NULL	0	NULL	UI	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	UI is common yet underreported by UAE women because of cultural attitudes and inadequate public knowledge .
	manualset3
196049	2	415984	7	NULL	NULL	0	NULL	UAE women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	UI is common yet underreported by UAE women because of cultural attitudes and inadequate public knowledge .
	manualset3
196050	3	415984	7	NULL	NULL	0	NULL	cultural attitudes	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	UI is common yet underreported by UAE women because of cultural attitudes and inadequate public knowledge .
	manualset3
196051	4	415984	7	NULL	NULL	0	NULL	inadequate public knowledge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	UI is common yet underreported by UAE women because of cultural attitudes and inadequate public knowledge .
	manualset3
196052	1	415985	7	NULL	NULL	0	NULL	UK hip fracture audit	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	UK hip fracture audit shows wide variation in standards of care .
	manualset3
196053	2	415985	7	NULL	NULL	0	NULL	wide variation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	UK hip fracture audit shows wide variation in standards of care .
	manualset3
196054	3	415985	7	NULL	NULL	0	NULL	standards	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	UK hip fracture audit shows wide variation in standards of care .
	manualset3
196055	4	415985	7	NULL	NULL	0	NULL	care	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	UK hip fracture audit shows wide variation in standards of care .
	manualset3
196056	1	415986	7	NULL	NULL	0	NULL	UL-5 A1-like antibodies	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	UL-5 A1-like antibodies against peptide/MHC complexes could prove valuable tools for research on T-cell recognition and MHC function .
	manualset3
196057	2	415986	7	NULL	NULL	0	NULL	peptide/MHC complexes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	UL-5 A1-like antibodies against peptide/MHC complexes could prove valuable tools for research on T-cell recognition and MHC function .
	manualset3
196058	3	415986	7	NULL	NULL	0	NULL	valuable tools	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	UL-5 A1-like antibodies against peptide/MHC complexes could prove valuable tools for research on T-cell recognition and MHC function .
	manualset3
196059	4	415986	7	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	UL-5 A1-like antibodies against peptide/MHC complexes could prove valuable tools for research on T-cell recognition and MHC function .
	manualset3
196060	5	415986	7	NULL	NULL	0	NULL	T-cell recognition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	UL-5 A1-like antibodies against peptide/MHC complexes could prove valuable tools for research on T-cell recognition and MHC function .
	manualset3
196061	6	415986	7	NULL	NULL	0	NULL	MHC function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	UL-5 A1-like antibodies against peptide/MHC complexes could prove valuable tools for research on T-cell recognition and MHC function .
	manualset3
196062	1	415987	7	NULL	NULL	0	NULL	US units	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	US units are commonly found in hospitals and clinics of all sizes , and a growing number of medical staff such as doctors and nurses are exposed to hand-transmitted ultrasound waves in their work-place .
	manualset3
196063	2	415987	7	NULL	NULL	0	NULL	 hospitals 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	US units are commonly found in hospitals and clinics of all sizes , and a growing number of medical staff such as doctors and nurses are exposed to hand-transmitted ultrasound waves in their work-place .
	manualset3
196064	3	415987	7	NULL	NULL	0	NULL	clinics	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	US units are commonly found in hospitals and clinics of all sizes , and a growing number of medical staff such as doctors and nurses are exposed to hand-transmitted ultrasound waves in their work-place .
	manualset3
196065	4	415987	7	NULL	NULL	0	NULL	sizes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	US units are commonly found in hospitals and clinics of all sizes , and a growing number of medical staff such as doctors and nurses are exposed to hand-transmitted ultrasound waves in their work-place .
	manualset3
196066	5	415987	7	NULL	NULL	0	NULL	growing number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	US units are commonly found in hospitals and clinics of all sizes , and a growing number of medical staff such as doctors and nurses are exposed to hand-transmitted ultrasound waves in their work-place .
	manualset3
196067	6	415987	7	NULL	NULL	0	NULL	medical staff	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	US units are commonly found in hospitals and clinics of all sizes , and a growing number of medical staff such as doctors and nurses are exposed to hand-transmitted ultrasound waves in their work-place .
	manualset3
196068	7	415987	7	NULL	NULL	0	NULL	doctors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	US units are commonly found in hospitals and clinics of all sizes , and a growing number of medical staff such as doctors and nurses are exposed to hand-transmitted ultrasound waves in their work-place .
	manualset3
196069	8	415987	7	NULL	NULL	0	NULL	nurses	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	US units are commonly found in hospitals and clinics of all sizes , and a growing number of medical staff such as doctors and nurses are exposed to hand-transmitted ultrasound waves in their work-place .
	manualset3
196070	9	415987	7	NULL	NULL	0	NULL	 hand-transmitted ultrasound waves	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	US units are commonly found in hospitals and clinics of all sizes , and a growing number of medical staff such as doctors and nurses are exposed to hand-transmitted ultrasound waves in their work-place .
	manualset3
196071	10	415987	7	NULL	NULL	0	NULL	work-place	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	US units are commonly found in hospitals and clinics of all sizes , and a growing number of medical staff such as doctors and nurses are exposed to hand-transmitted ultrasound waves in their work-place .
	manualset3
196072	1	415988	7	NULL	NULL	0	NULL	USAID research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	USAID research in developing countries has focused on three areas : 1 ) reducing common childhood illnesses , 2 ) reducing high reproductive morbidity and mortality , and 3 ) reducing the transmission of HIV/AIDS .
	manualset3
196073	2	415988	7	NULL	NULL	NULL	NULL	developing countries	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	USAID research in developing countries has focused on three areas : 1 ) reducing common childhood illnesses , 2 ) reducing high reproductive morbidity and mortality , and 3 ) reducing the transmission of HIV/AIDS .
	manualset3
196074	3	415988	7	NULL	NULL	0	NULL	three areas 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	USAID research in developing countries has focused on three areas : 1 ) reducing common childhood illnesses , 2 ) reducing high reproductive morbidity and mortality , and 3 ) reducing the transmission of HIV/AIDS .
	manualset3
196075	4	415988	7	NULL	NULL	0	NULL	childhood illnesses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	USAID research in developing countries has focused on three areas : 1 ) reducing common childhood illnesses , 2 ) reducing high reproductive morbidity and mortality , and 3 ) reducing the transmission of HIV/AIDS .
	manualset3
196076	5	415988	7	NULL	NULL	0	NULL	 high reproductive morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	USAID research in developing countries has focused on three areas : 1 ) reducing common childhood illnesses , 2 ) reducing high reproductive morbidity and mortality , and 3 ) reducing the transmission of HIV/AIDS .
	manualset3
196077	6	415988	7	NULL	NULL	0	NULL	high reproductive mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	USAID research in developing countries has focused on three areas : 1 ) reducing common childhood illnesses , 2 ) reducing high reproductive morbidity and mortality , and 3 ) reducing the transmission of HIV/AIDS .
	manualset3
196078	7	415988	7	NULL	NULL	0	NULL	transmission 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	USAID research in developing countries has focused on three areas : 1 ) reducing common childhood illnesses , 2 ) reducing high reproductive morbidity and mortality , and 3 ) reducing the transmission of HIV/AIDS .
	manualset3
196079	8	415988	7	NULL	NULL	0	NULL	HIV/AIDS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	USAID research in developing countries has focused on three areas : 1 ) reducing common childhood illnesses , 2 ) reducing high reproductive morbidity and mortality , and 3 ) reducing the transmission of HIV/AIDS .
	manualset3
198345	9	415988	7	NULL	NULL	0	NULL	reducing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	USAID research in developing countries has focused on three areas : 1 ) reducing common childhood illnesses , 2 ) reducing high reproductive morbidity and mortality , and 3 ) reducing the transmission of HIV/AIDS .
	manualset3
196080	1	415989	7	NULL	NULL	0	NULL	UV-irradiated cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	UV-irradiated cells also displayed a mutator phenotype towards untreated parvovirus H-1 .
	manualset3
196081	2	415989	7	NULL	NULL	0	NULL	mutator phenotype	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	UV-irradiated cells also displayed a mutator phenotype towards untreated parvovirus H-1 .
	manualset3
196082	3	415989	7	NULL	NULL	0	NULL	untreated parvovirus H-1	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	UV-irradiated cells also displayed a mutator phenotype towards untreated parvovirus H-1 .
	manualset3
196083	1	415990	7	NULL	NULL	0	NULL	six years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After six years of follow-up the aneurysm diameter has not changed and no complications were observed .
	manualset3
196084	2	415990	7	NULL	NULL	0	NULL	 follow-up	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After six years of follow-up the aneurysm diameter has not changed and no complications were observed .
	manualset3
196085	3	415990	7	NULL	NULL	0	NULL	aneurysm diameter	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After six years of follow-up the aneurysm diameter has not changed and no complications were observed .
	manualset3
196086	4	415990	7	NULL	NULL	0	NULL	 no complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After six years of follow-up the aneurysm diameter has not changed and no complications were observed .
	manualset3
196087	1	415991	7	NULL	NULL	0	NULL	UV-light-induced protein-DNA linkages	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	UV-light-induced protein-DNA linkages stabilize the structure of the preparation , whereas the action of chelate agents causes DNP-200 angstrom leads to DNP-100 angstrom transfer .
	manualset3
196088	2	415991	7	NULL	NULL	0	NULL	structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	UV-light-induced protein-DNA linkages stabilize the structure of the preparation , whereas the action of chelate agents causes DNP-200 angstrom leads to DNP-100 angstrom transfer .
	manualset3
196089	3	415991	7	NULL	NULL	0	NULL	preparation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	UV-light-induced protein-DNA linkages stabilize the structure of the preparation , whereas the action of chelate agents causes DNP-200 angstrom leads to DNP-100 angstrom transfer .
	manualset3
196090	4	415991	7	NULL	NULL	0	NULL	action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	UV-light-induced protein-DNA linkages stabilize the structure of the preparation , whereas the action of chelate agents causes DNP-200 angstrom leads to DNP-100 angstrom transfer .
	manualset3
196091	5	415991	7	NULL	NULL	0	NULL	chelate agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	UV-light-induced protein-DNA linkages stabilize the structure of the preparation , whereas the action of chelate agents causes DNP-200 angstrom leads to DNP-100 angstrom transfer .
	manualset3
196092	6	415991	7	NULL	NULL	0	NULL	DNP-200 angstrom	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	UV-light-induced protein-DNA linkages stabilize the structure of the preparation , whereas the action of chelate agents causes DNP-200 angstrom leads to DNP-100 angstrom transfer .
	manualset3
196093	7	415991	7	NULL	NULL	0	NULL	DNP-100 angstrom transfer	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	UV-light-induced protein-DNA linkages stabilize the structure of the preparation , whereas the action of chelate agents causes DNP-200 angstrom leads to DNP-100 angstrom transfer .
	manualset3
196094	1	415992	7	NULL	NULL	0	NULL	UV-radiation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	UV-radiation suppressed endogenous stimulants of indole nature .
	manualset3
196095	2	415992	7	NULL	NULL	0	NULL	endogenous stimulants	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	UV-radiation suppressed endogenous stimulants of indole nature .
	manualset3
196096	3	415992	7	NULL	NULL	0	NULL	indole nature	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	UV-radiation suppressed endogenous stimulants of indole nature .
	manualset3
196097	1	415993	7	NULL	NULL	0	NULL	UV irradiation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	UV irradiation did not increase DEL recombination frequencies in G1 or G2 , whereas gamma-rays increased DEL recombination frequencies in both phases .
	manualset3
196098	2	415993	7	NULL	NULL	0	NULL	DEL recombination frequencies	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	UV irradiation did not increase DEL recombination frequencies in G1 or G2 , whereas gamma-rays increased DEL recombination frequencies in both phases .
	manualset3
196099	3	415993	7	NULL	NULL	NULL	NULL	G1	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	UV irradiation did not increase DEL recombination frequencies in G1 or G2 , whereas gamma-rays increased DEL recombination frequencies in both phases .
	manualset3
196100	4	415993	7	NULL	NULL	NULL	NULL	G2	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	UV irradiation did not increase DEL recombination frequencies in G1 or G2 , whereas gamma-rays increased DEL recombination frequencies in both phases .
	manualset3
196101	5	415993	7	NULL	NULL	0	NULL	gamma-rays	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	UV irradiation did not increase DEL recombination frequencies in G1 or G2 , whereas gamma-rays increased DEL recombination frequencies in both phases .
	manualset3
196102	6	415993	7	NULL	NULL	0	NULL	DEL recombination frequencies	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	UV irradiation did not increase DEL recombination frequencies in G1 or G2 , whereas gamma-rays increased DEL recombination frequencies in both phases .
	manualset3
196103	7	415993	7	NULL	NULL	0	NULL	phases	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	UV irradiation did not increase DEL recombination frequencies in G1 or G2 , whereas gamma-rays increased DEL recombination frequencies in both phases .
	manualset3
196104	1	415994	7	NULL	NULL	NULL	NULL	UV transmission	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	UV transmission and the sun protection factor ( SPF ) were assessed for different cream formulations .
	manualset3
196105	2	415994	7	NULL	NULL	NULL	NULL	sun protection factor ( SPF )	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	UV transmission and the sun protection factor ( SPF ) were assessed for different cream formulations .
	manualset3
196106	3	415994	7	NULL	NULL	NULL	NULL	cream formulations	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	UV transmission and the sun protection factor ( SPF ) were assessed for different cream formulations .
	manualset3
196107	1	415995	7	NULL	NULL	NULL	NULL	UVB-treated allografts	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	UVB-treated allografts showed MHC class II antigen expression labeling of 20 % of the endothelial cells .
	manualset3
196108	2	415995	7	NULL	NULL	NULL	NULL	MHC class II antigen expression labeling	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	UVB-treated allografts showed MHC class II antigen expression labeling of 20 % of the endothelial cells .
	manualset3
196109	3	415995	7	NULL	NULL	0	NULL	20 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	UVB-treated allografts showed MHC class II antigen expression labeling of 20 % of the endothelial cells .
	manualset3
196110	4	415995	7	NULL	NULL	0	NULL	endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	UVB-treated allografts showed MHC class II antigen expression labeling of 20 % of the endothelial cells .
	manualset3
196111	1	415996	7	NULL	NULL	0	NULL	UVB phototherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	UVB phototherapy is widely used for the treatment of psoriasis and atopic dermatitis , however , only limited reports evaluate its usefulness in the treatment of mycosis fungoides .
	manualset3
196112	2	415996	7	NULL	NULL	0	NULL	 treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	UVB phototherapy is widely used for the treatment of psoriasis and atopic dermatitis , however , only limited reports evaluate its usefulness in the treatment of mycosis fungoides .
	manualset3
196113	3	415996	7	NULL	NULL	0	NULL	psoriasis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	UVB phototherapy is widely used for the treatment of psoriasis and atopic dermatitis , however , only limited reports evaluate its usefulness in the treatment of mycosis fungoides .
	manualset3
196114	4	415996	7	NULL	NULL	0	NULL	atopic dermatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	UVB phototherapy is widely used for the treatment of psoriasis and atopic dermatitis , however , only limited reports evaluate its usefulness in the treatment of mycosis fungoides .
	manualset3
196115	5	415996	7	NULL	NULL	0	NULL	limited reports	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	UVB phototherapy is widely used for the treatment of psoriasis and atopic dermatitis , however , only limited reports evaluate its usefulness in the treatment of mycosis fungoides .
	manualset3
196116	6	415996	7	NULL	NULL	0	NULL	 treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	UVB phototherapy is widely used for the treatment of psoriasis and atopic dermatitis , however , only limited reports evaluate its usefulness in the treatment of mycosis fungoides .
	manualset3
196117	7	415996	7	NULL	NULL	0	NULL	mycosis fungoides	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	UVB phototherapy is widely used for the treatment of psoriasis and atopic dermatitis , however , only limited reports evaluate its usefulness in the treatment of mycosis fungoides .
	manualset3
196118	1	415997	7	NULL	NULL	0	NULL	UVR	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	UVR administered to pre-sensitised mice regulated allergen responsiveness by cells from the airway draining lymph nodes only with a sensitisation protocol involving allergen and adjuvant at 5 % strength of the original dose ( 1 g OVA in 0.2 mg alum/mouse ) .
	manualset3
196119	2	415997	7	NULL	NULL	0	NULL	pre-sensitised mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	UVR administered to pre-sensitised mice regulated allergen responsiveness by cells from the airway draining lymph nodes only with a sensitisation protocol involving allergen and adjuvant at 5 % strength of the original dose ( 1 g OVA in 0.2 mg alum/mouse ) .
	manualset3
196120	3	415997	7	NULL	NULL	0	NULL	allergen responsiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	UVR administered to pre-sensitised mice regulated allergen responsiveness by cells from the airway draining lymph nodes only with a sensitisation protocol involving allergen and adjuvant at 5 % strength of the original dose ( 1 g OVA in 0.2 mg alum/mouse ) .
	manualset3
196121	4	415997	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	UVR administered to pre-sensitised mice regulated allergen responsiveness by cells from the airway draining lymph nodes only with a sensitisation protocol involving allergen and adjuvant at 5 % strength of the original dose ( 1 g OVA in 0.2 mg alum/mouse ) .
	manualset3
196122	5	415997	7	NULL	NULL	0	NULL	airway	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	UVR administered to pre-sensitised mice regulated allergen responsiveness by cells from the airway draining lymph nodes only with a sensitisation protocol involving allergen and adjuvant at 5 % strength of the original dose ( 1 g OVA in 0.2 mg alum/mouse ) .
	manualset3
196123	6	415997	7	NULL	NULL	0	NULL	lymph nodes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	UVR administered to pre-sensitised mice regulated allergen responsiveness by cells from the airway draining lymph nodes only with a sensitisation protocol involving allergen and adjuvant at 5 % strength of the original dose ( 1 g OVA in 0.2 mg alum/mouse ) .
	manualset3
196124	7	415997	7	NULL	NULL	0	NULL	sensitisation protocol 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	UVR administered to pre-sensitised mice regulated allergen responsiveness by cells from the airway draining lymph nodes only with a sensitisation protocol involving allergen and adjuvant at 5 % strength of the original dose ( 1 g OVA in 0.2 mg alum/mouse ) .
	manualset3
196125	8	415997	7	NULL	NULL	0	NULL	allergen	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	UVR administered to pre-sensitised mice regulated allergen responsiveness by cells from the airway draining lymph nodes only with a sensitisation protocol involving allergen and adjuvant at 5 % strength of the original dose ( 1 g OVA in 0.2 mg alum/mouse ) .
	manualset3
196126	9	415997	7	NULL	NULL	0	NULL	adjuvant	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	UVR administered to pre-sensitised mice regulated allergen responsiveness by cells from the airway draining lymph nodes only with a sensitisation protocol involving allergen and adjuvant at 5 % strength of the original dose ( 1 g OVA in 0.2 mg alum/mouse ) .
	manualset3
196127	10	415997	7	NULL	NULL	0	NULL	5 % strength	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	UVR administered to pre-sensitised mice regulated allergen responsiveness by cells from the airway draining lymph nodes only with a sensitisation protocol involving allergen and adjuvant at 5 % strength of the original dose ( 1 g OVA in 0.2 mg alum/mouse ) .
	manualset3
196128	11	415997	7	NULL	NULL	0	NULL	original dose	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	UVR administered to pre-sensitised mice regulated allergen responsiveness by cells from the airway draining lymph nodes only with a sensitisation protocol involving allergen and adjuvant at 5 % strength of the original dose ( 1 g OVA in 0.2 mg alum/mouse ) .
	manualset3
196129	12	415997	7	NULL	NULL	0	NULL	1 g OVA	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	UVR administered to pre-sensitised mice regulated allergen responsiveness by cells from the airway draining lymph nodes only with a sensitisation protocol involving allergen and adjuvant at 5 % strength of the original dose ( 1 g OVA in 0.2 mg alum/mouse ) .
	manualset3
196130	13	415997	7	NULL	NULL	0	NULL	 0.2 mg alum/mouse	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	UVR administered to pre-sensitised mice regulated allergen responsiveness by cells from the airway draining lymph nodes only with a sensitisation protocol involving allergen and adjuvant at 5 % strength of the original dose ( 1 g OVA in 0.2 mg alum/mouse ) .
	manualset3
196131	1	415998	7	NULL	NULL	NULL	NULL	UVS cones	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	UVS cones subsequently reappear in the retina near sexual maturation and the return migration to natal streams .
	manualset3
196132	2	415998	7	NULL	NULL	0	NULL	retina	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	UVS cones subsequently reappear in the retina near sexual maturation and the return migration to natal streams .
	manualset3
196133	3	415998	7	NULL	NULL	0	NULL	sexual maturation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	UVS cones subsequently reappear in the retina near sexual maturation and the return migration to natal streams .
	manualset3
196134	4	415998	7	NULL	NULL	0	NULL	migration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	UVS cones subsequently reappear in the retina near sexual maturation and the return migration to natal streams .
	manualset3
196135	5	415998	7	NULL	NULL	0	NULL	natal streams	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	UVS cones subsequently reappear in the retina near sexual maturation and the return migration to natal streams .
	manualset3
196136	1	415999	7	NULL	NULL	0	NULL	bleeding 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After stopping the bleeding from the mucosal defect by injection therapy in one patient , the further course was uneventful in both .
	manualset3
196137	2	415999	7	NULL	NULL	0	NULL	mucosal defect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After stopping the bleeding from the mucosal defect by injection therapy in one patient , the further course was uneventful in both .
	manualset3
196138	3	415999	7	NULL	NULL	0	NULL	injection therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After stopping the bleeding from the mucosal defect by injection therapy in one patient , the further course was uneventful in both .
	manualset3
196139	4	415999	7	NULL	NULL	0	NULL	one patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	After stopping the bleeding from the mucosal defect by injection therapy in one patient , the further course was uneventful in both .
	manualset3
196140	5	415999	7	NULL	NULL	0	NULL	course	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After stopping the bleeding from the mucosal defect by injection therapy in one patient , the further course was uneventful in both .
	manualset3
196141	1	416000	7	NULL	NULL	0	NULL	Ubiquitin ligase Smurf1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Ubiquitin ligase Smurf1 mediates tumor necrosis factor-induced systemic bone loss by promoting proteasomal degradation of bone morphogenetic signaling proteins .
	manualset3
196142	2	416000	7	NULL	NULL	0	NULL	tumor necrosis factor-induced systemic bone loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ubiquitin ligase Smurf1 mediates tumor necrosis factor-induced systemic bone loss by promoting proteasomal degradation of bone morphogenetic signaling proteins .
	manualset3
196143	3	416000	7	NULL	NULL	0	NULL	proteasomal degradation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ubiquitin ligase Smurf1 mediates tumor necrosis factor-induced systemic bone loss by promoting proteasomal degradation of bone morphogenetic signaling proteins .
	manualset3
196144	4	416000	7	NULL	NULL	0	NULL	bone morphogenetic signaling proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ubiquitin ligase Smurf1 mediates tumor necrosis factor-induced systemic bone loss by promoting proteasomal degradation of bone morphogenetic signaling proteins .
	manualset3
196145	1	416001	7	NULL	NULL	0	NULL	Ubiquitination	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ubiquitination of Plk1 by Chfr delayed the activation of the Cdc25C phosphatase and the inactivation of the Weel kinase , leading to a delay in Cdc 2 activation .
	manualset3
196146	2	416001	7	NULL	NULL	0	NULL	Plk1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Ubiquitination of Plk1 by Chfr delayed the activation of the Cdc25C phosphatase and the inactivation of the Weel kinase , leading to a delay in Cdc 2 activation .
	manualset3
196147	3	416001	7	NULL	NULL	0	NULL	Chfr	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Ubiquitination of Plk1 by Chfr delayed the activation of the Cdc25C phosphatase and the inactivation of the Weel kinase , leading to a delay in Cdc 2 activation .
	manualset3
196148	4	416001	7	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ubiquitination of Plk1 by Chfr delayed the activation of the Cdc25C phosphatase and the inactivation of the Weel kinase , leading to a delay in Cdc 2 activation .
	manualset3
196149	5	416001	7	NULL	NULL	0	NULL	Cdc25C phosphatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Ubiquitination of Plk1 by Chfr delayed the activation of the Cdc25C phosphatase and the inactivation of the Weel kinase , leading to a delay in Cdc 2 activation .
	manualset3
196150	6	416001	7	NULL	NULL	0	NULL	inactivation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ubiquitination of Plk1 by Chfr delayed the activation of the Cdc25C phosphatase and the inactivation of the Weel kinase , leading to a delay in Cdc 2 activation .
	manualset3
196151	7	416001	7	NULL	NULL	0	NULL	Weel kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Ubiquitination of Plk1 by Chfr delayed the activation of the Cdc25C phosphatase and the inactivation of the Weel kinase , leading to a delay in Cdc 2 activation .
	manualset3
196152	8	416001	7	NULL	NULL	0	NULL	 delay	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Ubiquitination of Plk1 by Chfr delayed the activation of the Cdc25C phosphatase and the inactivation of the Weel kinase , leading to a delay in Cdc 2 activation .
	manualset3
196153	9	416001	7	NULL	NULL	0	NULL	Cdc 2 activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ubiquitination of Plk1 by Chfr delayed the activation of the Cdc25C phosphatase and the inactivation of the Weel kinase , leading to a delay in Cdc 2 activation .
	manualset3
196154	1	416002	7	NULL	NULL	0	NULL	Ulcer suturing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ulcer suturing was carried out in 226 patients ( 87.6 % ) , the rest were subjected to other operations .
	manualset3
196155	2	416002	7	NULL	NULL	0	NULL	226 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ulcer suturing was carried out in 226 patients ( 87.6 % ) , the rest were subjected to other operations .
	manualset3
196156	3	416002	7	NULL	NULL	0	NULL	87.6 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ulcer suturing was carried out in 226 patients ( 87.6 % ) , the rest were subjected to other operations .
	manualset3
196157	4	416002	7	NULL	NULL	0	NULL	operations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ulcer suturing was carried out in 226 patients ( 87.6 % ) , the rest were subjected to other operations .
	manualset3
196158	1	416003	7	NULL	NULL	0	NULL	 understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultimately , a better understanding of the regulatory mechanisms involved in beta-carotene overproduction will facilitate innovative production of specific carotenoids and other products in D. salina and in related organisms .
	manualset3
196159	2	416003	7	NULL	NULL	NULL	NULL	regulatory mechanisms	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ultimately , a better understanding of the regulatory mechanisms involved in beta-carotene overproduction will facilitate innovative production of specific carotenoids and other products in D. salina and in related organisms .
	manualset3
196160	3	416003	7	NULL	NULL	NULL	NULL	beta-carotene overproduction	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ultimately , a better understanding of the regulatory mechanisms involved in beta-carotene overproduction will facilitate innovative production of specific carotenoids and other products in D. salina and in related organisms .
	manualset3
196161	4	416003	7	NULL	NULL	0	NULL	innovative production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultimately , a better understanding of the regulatory mechanisms involved in beta-carotene overproduction will facilitate innovative production of specific carotenoids and other products in D. salina and in related organisms .
	manualset3
196162	5	416003	7	NULL	NULL	0	NULL	carotenoids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultimately , a better understanding of the regulatory mechanisms involved in beta-carotene overproduction will facilitate innovative production of specific carotenoids and other products in D. salina and in related organisms .
	manualset3
196163	6	416003	7	NULL	NULL	0	NULL	D. salina	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultimately , a better understanding of the regulatory mechanisms involved in beta-carotene overproduction will facilitate innovative production of specific carotenoids and other products in D. salina and in related organisms .
	manualset3
196164	7	416003	7	NULL	NULL	0	NULL	 organisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultimately , a better understanding of the regulatory mechanisms involved in beta-carotene overproduction will facilitate innovative production of specific carotenoids and other products in D. salina and in related organisms .
	manualset3
197256	8	416003	7	NULL	NULL	0	NULL	 products	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultimately , a better understanding of the regulatory mechanisms involved in beta-carotene overproduction will facilitate innovative production of specific carotenoids and other products in D. salina and in related organisms .
	manualset3
196165	1	416004	7	NULL	NULL	0	NULL	 trial data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultimately , more trial data may be necessary to substantiate the increased use of distal protection devices in infrainguinal interventions to justify the increase in cost , complexity , and potential risks associated with the use of this technology .
	manualset3
196166	2	416004	7	NULL	NULL	0	NULL	distal protection devices	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultimately , more trial data may be necessary to substantiate the increased use of distal protection devices in infrainguinal interventions to justify the increase in cost , complexity , and potential risks associated with the use of this technology .
	manualset3
196167	3	416004	7	NULL	NULL	0	NULL	 increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultimately , more trial data may be necessary to substantiate the increased use of distal protection devices in infrainguinal interventions to justify the increase in cost , complexity , and potential risks associated with the use of this technology .
	manualset3
196168	4	416004	7	NULL	NULL	0	NULL	cost	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultimately , more trial data may be necessary to substantiate the increased use of distal protection devices in infrainguinal interventions to justify the increase in cost , complexity , and potential risks associated with the use of this technology .
	manualset3
196169	5	416004	7	NULL	NULL	0	NULL	complexity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultimately , more trial data may be necessary to substantiate the increased use of distal protection devices in infrainguinal interventions to justify the increase in cost , complexity , and potential risks associated with the use of this technology .
	manualset3
196170	6	416004	7	NULL	NULL	0	NULL	potential risks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultimately , more trial data may be necessary to substantiate the increased use of distal protection devices in infrainguinal interventions to justify the increase in cost , complexity , and potential risks associated with the use of this technology .
	manualset3
196171	7	416004	7	NULL	NULL	0	NULL	 technology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultimately , more trial data may be necessary to substantiate the increased use of distal protection devices in infrainguinal interventions to justify the increase in cost , complexity , and potential risks associated with the use of this technology .
	manualset3
196172	8	416004	7	NULL	NULL	0	NULL	 infrainguinal interventions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultimately , more trial data may be necessary to substantiate the increased use of distal protection devices in infrainguinal interventions to justify the increase in cost , complexity , and potential risks associated with the use of this technology .
	manualset3
196173	1	416005	7	NULL	NULL	0	NULL	Ultradian `` oscillations ''	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultradian `` oscillations '' or `` pulses '' of insulin secretion with periods around 120 min occur in man .
	manualset3
196174	2	416005	7	NULL	NULL	0	NULL	 `` pulses ''	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultradian `` oscillations '' or `` pulses '' of insulin secretion with periods around 120 min occur in man .
	manualset3
196175	3	416005	7	NULL	NULL	0	NULL	insulin secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultradian `` oscillations '' or `` pulses '' of insulin secretion with periods around 120 min occur in man .
	manualset3
196176	4	416005	7	NULL	NULL	0	NULL	 periods	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultradian `` oscillations '' or `` pulses '' of insulin secretion with periods around 120 min occur in man .
	manualset3
196177	5	416005	7	NULL	NULL	0	NULL	120 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultradian `` oscillations '' or `` pulses '' of insulin secretion with periods around 120 min occur in man .
	manualset3
196178	6	416005	7	NULL	NULL	0	NULL	man	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultradian `` oscillations '' or `` pulses '' of insulin secretion with periods around 120 min occur in man .
	manualset3
196179	1	416006	7	NULL	NULL	0	NULL	Ultrahigh-contrast and wideband nanoscale photonic crystal	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrahigh-contrast and wideband nanoscale photonic crystal all-optical diode .
	manualset3
196180	2	416006	7	NULL	NULL	0	NULL	all-optical diode	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrahigh-contrast and wideband nanoscale photonic crystal all-optical diode .
	manualset3
196181	1	416007	7	NULL	NULL	0	NULL	Ultrahigh frequency acoustic resonances 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrahigh frequency acoustic resonances ( approximately 2 GHz ) trapped within the glass core ( approximately 1 microm diameter ) of a photonic crystal fiber are selectively excited through electrostriction using laser pulses of duration 100 ps and energy 500 pJ .
	manualset3
196182	2	416007	7	NULL	NULL	0	NULL	2 GHz	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrahigh frequency acoustic resonances ( approximately 2 GHz ) trapped within the glass core ( approximately 1 microm diameter ) of a photonic crystal fiber are selectively excited through electrostriction using laser pulses of duration 100 ps and energy 500 pJ .
	manualset3
196183	3	416007	7	NULL	NULL	0	NULL	glass core	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrahigh frequency acoustic resonances ( approximately 2 GHz ) trapped within the glass core ( approximately 1 microm diameter ) of a photonic crystal fiber are selectively excited through electrostriction using laser pulses of duration 100 ps and energy 500 pJ .
	manualset3
196184	4	416007	7	NULL	NULL	0	NULL	1 microm diameter 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrahigh frequency acoustic resonances ( approximately 2 GHz ) trapped within the glass core ( approximately 1 microm diameter ) of a photonic crystal fiber are selectively excited through electrostriction using laser pulses of duration 100 ps and energy 500 pJ .
	manualset3
196185	5	416007	7	NULL	NULL	0	NULL	photonic crystal fiber	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrahigh frequency acoustic resonances ( approximately 2 GHz ) trapped within the glass core ( approximately 1 microm diameter ) of a photonic crystal fiber are selectively excited through electrostriction using laser pulses of duration 100 ps and energy 500 pJ .
	manualset3
196186	6	416007	7	NULL	NULL	0	NULL	electrostriction	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrahigh frequency acoustic resonances ( approximately 2 GHz ) trapped within the glass core ( approximately 1 microm diameter ) of a photonic crystal fiber are selectively excited through electrostriction using laser pulses of duration 100 ps and energy 500 pJ .
	manualset3
196187	7	416007	7	NULL	NULL	0	NULL	laser pulses	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrahigh frequency acoustic resonances ( approximately 2 GHz ) trapped within the glass core ( approximately 1 microm diameter ) of a photonic crystal fiber are selectively excited through electrostriction using laser pulses of duration 100 ps and energy 500 pJ .
	manualset3
196188	8	416007	7	NULL	NULL	0	NULL	duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrahigh frequency acoustic resonances ( approximately 2 GHz ) trapped within the glass core ( approximately 1 microm diameter ) of a photonic crystal fiber are selectively excited through electrostriction using laser pulses of duration 100 ps and energy 500 pJ .
	manualset3
196189	9	416007	7	NULL	NULL	0	NULL	100 ps	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrahigh frequency acoustic resonances ( approximately 2 GHz ) trapped within the glass core ( approximately 1 microm diameter ) of a photonic crystal fiber are selectively excited through electrostriction using laser pulses of duration 100 ps and energy 500 pJ .
	manualset3
196190	10	416007	7	NULL	NULL	0	NULL	energy	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrahigh frequency acoustic resonances ( approximately 2 GHz ) trapped within the glass core ( approximately 1 microm diameter ) of a photonic crystal fiber are selectively excited through electrostriction using laser pulses of duration 100 ps and energy 500 pJ .
	manualset3
196191	11	416007	7	NULL	NULL	0	NULL	500 pJ 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrahigh frequency acoustic resonances ( approximately 2 GHz ) trapped within the glass core ( approximately 1 microm diameter ) of a photonic crystal fiber are selectively excited through electrostriction using laser pulses of duration 100 ps and energy 500 pJ .
	manualset3
196192	1	416008	7	NULL	NULL	0	NULL	 surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After surgery , patients with valvular disease showed a decrease in respiratory system and lung resistances .
	manualset3
196193	2	416008	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	After surgery , patients with valvular disease showed a decrease in respiratory system and lung resistances .
	manualset3
196194	3	416008	7	NULL	NULL	0	NULL	valvular disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	After surgery , patients with valvular disease showed a decrease in respiratory system and lung resistances .
	manualset3
196195	4	416008	7	NULL	NULL	0	NULL	respiratory system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After surgery , patients with valvular disease showed a decrease in respiratory system and lung resistances .
	manualset3
196196	5	416008	7	NULL	NULL	0	NULL	lung resistances	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After surgery , patients with valvular disease showed a decrease in respiratory system and lung resistances .
	manualset3
196197	1	416009	7	NULL	NULL	0	NULL	Ultrashort pulsed lasers	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrashort pulsed lasers , operating through the phenomenon of mode-locking , have had a significant role in many facets of our society for 50 years , for example , in the way we exchange information , measure and diagnose diseases , process materials , and in many other applications .
	manualset3
196198	2	416009	7	NULL	NULL	0	NULL	phenomenon	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrashort pulsed lasers , operating through the phenomenon of mode-locking , have had a significant role in many facets of our society for 50 years , for example , in the way we exchange information , measure and diagnose diseases , process materials , and in many other applications .
	manualset3
196199	3	416009	7	NULL	NULL	0	NULL	mode-locking	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrashort pulsed lasers , operating through the phenomenon of mode-locking , have had a significant role in many facets of our society for 50 years , for example , in the way we exchange information , measure and diagnose diseases , process materials , and in many other applications .
	manualset3
196200	4	416009	7	NULL	NULL	NULL	NULL	role	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ultrashort pulsed lasers , operating through the phenomenon of mode-locking , have had a significant role in many facets of our society for 50 years , for example , in the way we exchange information , measure and diagnose diseases , process materials , and in many other applications .
	manualset3
196201	5	416009	7	NULL	NULL	0	NULL	many facets 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrashort pulsed lasers , operating through the phenomenon of mode-locking , have had a significant role in many facets of our society for 50 years , for example , in the way we exchange information , measure and diagnose diseases , process materials , and in many other applications .
	manualset3
196202	6	416009	7	NULL	NULL	0	NULL	society	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrashort pulsed lasers , operating through the phenomenon of mode-locking , have had a significant role in many facets of our society for 50 years , for example , in the way we exchange information , measure and diagnose diseases , process materials , and in many other applications .
	manualset3
196203	7	416009	7	NULL	NULL	0	NULL	50 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrashort pulsed lasers , operating through the phenomenon of mode-locking , have had a significant role in many facets of our society for 50 years , for example , in the way we exchange information , measure and diagnose diseases , process materials , and in many other applications .
	manualset3
196204	8	416009	7	NULL	NULL	0	NULL	example	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrashort pulsed lasers , operating through the phenomenon of mode-locking , have had a significant role in many facets of our society for 50 years , for example , in the way we exchange information , measure and diagnose diseases , process materials , and in many other applications .
	manualset3
196205	9	416009	7	NULL	NULL	0	NULL	information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrashort pulsed lasers , operating through the phenomenon of mode-locking , have had a significant role in many facets of our society for 50 years , for example , in the way we exchange information , measure and diagnose diseases , process materials , and in many other applications .
	manualset3
196206	10	416009	7	NULL	NULL	0	NULL	 diseases 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrashort pulsed lasers , operating through the phenomenon of mode-locking , have had a significant role in many facets of our society for 50 years , for example , in the way we exchange information , measure and diagnose diseases , process materials , and in many other applications .
	manualset3
196207	11	416009	7	NULL	NULL	0	NULL	process materials	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrashort pulsed lasers , operating through the phenomenon of mode-locking , have had a significant role in many facets of our society for 50 years , for example , in the way we exchange information , measure and diagnose diseases , process materials , and in many other applications .
	manualset3
196208	12	416009	7	NULL	NULL	0	NULL	 applications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrashort pulsed lasers , operating through the phenomenon of mode-locking , have had a significant role in many facets of our society for 50 years , for example , in the way we exchange information , measure and diagnose diseases , process materials , and in many other applications .
	manualset3
196209	1	416010	7	NULL	NULL	0	NULL	Ultrasonic imaging 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasonic imaging and oculoplethysmography in diagnosis of carotid occlusive disease .
	manualset3
196210	2	416010	7	NULL	NULL	0	NULL	oculoplethysmography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasonic imaging and oculoplethysmography in diagnosis of carotid occlusive disease .
	manualset3
196211	3	416010	7	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasonic imaging and oculoplethysmography in diagnosis of carotid occlusive disease .
	manualset3
196212	4	416010	7	NULL	NULL	0	NULL	carotid occlusive disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasonic imaging and oculoplethysmography in diagnosis of carotid occlusive disease .
	manualset3
196213	1	416011	7	NULL	NULL	0	NULL	Ultrasonic technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasonic technique for imaging tissue vibrations : preliminary results .
	manualset3
196214	2	416011	7	NULL	NULL	NULL	NULL	 tissue vibrations	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ultrasonic technique for imaging tissue vibrations : preliminary results .
	manualset3
196215	3	416011	7	NULL	NULL	0	NULL	preliminary results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasonic technique for imaging tissue vibrations : preliminary results .
	manualset3
196216	1	416012	7	NULL	NULL	0	NULL	Ultrasonography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasonography showed that the SPN became subcutaneous between S3 and S4 .
	manualset3
196217	2	416012	7	NULL	NULL	0	NULL	 SPN	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasonography showed that the SPN became subcutaneous between S3 and S4 .
	manualset3
196218	3	416012	7	NULL	NULL	0	NULL	subcutaneous 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasonography showed that the SPN became subcutaneous between S3 and S4 .
	manualset3
196219	4	416012	7	NULL	NULL	0	NULL	S3	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasonography showed that the SPN became subcutaneous between S3 and S4 .
	manualset3
196220	5	416012	7	NULL	NULL	0	NULL	S4	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasonography showed that the SPN became subcutaneous between S3 and S4 .
	manualset3
196221	1	416013	7	NULL	NULL	0	NULL	Ultrasound-assisted oxidative process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound-assisted oxidative process for sulfur removal from petroleum product feedstock .
	manualset3
196222	2	416013	7	NULL	NULL	0	NULL	sulfur removal 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound-assisted oxidative process for sulfur removal from petroleum product feedstock .
	manualset3
196223	3	416013	7	NULL	NULL	0	NULL	 petroleum product feedstock	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound-assisted oxidative process for sulfur removal from petroleum product feedstock .
	manualset3
196224	1	416014	7	NULL	NULL	0	NULL	Ultrasound-guided plexus anaesthesia	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound-guided plexus anaesthesia is markedly more effective than the blind technique when performed by a hand surgeon .
	manualset3
196225	2	416014	7	NULL	NULL	0	NULL	blind technique	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound-guided plexus anaesthesia is markedly more effective than the blind technique when performed by a hand surgeon .
	manualset3
196226	3	416014	7	NULL	NULL	0	NULL	hand surgeon	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound-guided plexus anaesthesia is markedly more effective than the blind technique when performed by a hand surgeon .
	manualset3
196227	1	416015	7	NULL	NULL	0	NULL	Ultrasound-induced free-radical production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound-induced free-radical production was significantly decreased at 1 mM and became undetectable at 2 mM CO ( 2 ) .
	manualset3
196228	2	416015	7	NULL	NULL	0	NULL	1 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound-induced free-radical production was significantly decreased at 1 mM and became undetectable at 2 mM CO ( 2 ) .
	manualset3
196229	3	416015	7	NULL	NULL	0	NULL	2 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound-induced free-radical production was significantly decreased at 1 mM and became undetectable at 2 mM CO ( 2 ) .
	manualset3
196230	4	416015	7	NULL	NULL	0	NULL	CO ( 2 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound-induced free-radical production was significantly decreased at 1 mM and became undetectable at 2 mM CO ( 2 ) .
	manualset3
196231	1	416016	7	NULL	NULL	0	NULL	surgical resection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After surgical resection of the abscess and under high-dose therapy with penicillin G the further course of disease was uneventful .
	manualset3
196232	2	416016	7	NULL	NULL	0	NULL	abscess	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After surgical resection of the abscess and under high-dose therapy with penicillin G the further course of disease was uneventful .
	manualset3
196233	3	416016	7	NULL	NULL	0	NULL	high-dose therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After surgical resection of the abscess and under high-dose therapy with penicillin G the further course of disease was uneventful .
	manualset3
196234	4	416016	7	NULL	NULL	0	NULL	penicillin G	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	After surgical resection of the abscess and under high-dose therapy with penicillin G the further course of disease was uneventful .
	manualset3
196235	5	416016	7	NULL	NULL	0	NULL	 course	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After surgical resection of the abscess and under high-dose therapy with penicillin G the further course of disease was uneventful .
	manualset3
196236	6	416016	7	NULL	NULL	0	NULL	 disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	After surgical resection of the abscess and under high-dose therapy with penicillin G the further course of disease was uneventful .
	manualset3
196238	1	416017	7	NULL	NULL	0	NULL	Ultrasound	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound for breast cancer screening and staging .
	manualset3
196239	2	416017	7	NULL	NULL	0	NULL	breast cancer screening	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound for breast cancer screening and staging .
	manualset3
196240	3	416017	7	NULL	NULL	0	NULL	breast cancer staging	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound for breast cancer screening and staging .
	manualset3
196241	1	416018	7	NULL	NULL	0	NULL	Ultrasound guided percutaneous fine needle aspiration biopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound guided percutaneous fine needle aspiration biopsy of focal liver lesions .
	manualset3
196242	2	416018	7	NULL	NULL	0	NULL	focal liver lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound guided percutaneous fine needle aspiration biopsy of focal liver lesions .
	manualset3
196243	1	416019	7	NULL	NULL	0	NULL	Ultrasound images	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound images allowed determination of the region over the women 's abdomen nearest to the fetal head , over which both the acoustic stimulator and the MEG sensors were subsequently placed .
	manualset3
196244	2	416019	7	NULL	NULL	0	NULL	determination 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound images allowed determination of the region over the women 's abdomen nearest to the fetal head , over which both the acoustic stimulator and the MEG sensors were subsequently placed .
	manualset3
196245	3	416019	7	NULL	NULL	0	NULL	region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound images allowed determination of the region over the women 's abdomen nearest to the fetal head , over which both the acoustic stimulator and the MEG sensors were subsequently placed .
	manualset3
196246	4	416019	7	NULL	NULL	0	NULL	women 's abdomen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound images allowed determination of the region over the women 's abdomen nearest to the fetal head , over which both the acoustic stimulator and the MEG sensors were subsequently placed .
	manualset3
196247	5	416019	7	NULL	NULL	0	NULL	fetal head	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound images allowed determination of the region over the women 's abdomen nearest to the fetal head , over which both the acoustic stimulator and the MEG sensors were subsequently placed .
	manualset3
196248	6	416019	7	NULL	NULL	0	NULL	acoustic stimulator	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound images allowed determination of the region over the women 's abdomen nearest to the fetal head , over which both the acoustic stimulator and the MEG sensors were subsequently placed .
	manualset3
196249	7	416019	7	NULL	NULL	0	NULL	MEG sensors 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound images allowed determination of the region over the women 's abdomen nearest to the fetal head , over which both the acoustic stimulator and the MEG sensors were subsequently placed .
	manualset3
196274	1	416020	7	NULL	NULL	0	NULL	Ultrastructural analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural analyses of the attachment ( bonding ) zone between bone and implanted biomaterials .
	manualset3
196275	2	416020	7	NULL	NULL	0	NULL	attachment ( bonding ) zone	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural analyses of the attachment ( bonding ) zone between bone and implanted biomaterials .
	manualset3
196276	3	416020	7	NULL	NULL	0	NULL	bone	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural analyses of the attachment ( bonding ) zone between bone and implanted biomaterials .
	manualset3
196277	4	416020	7	NULL	NULL	0	NULL	implanted biomaterials	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural analyses of the attachment ( bonding ) zone between bone and implanted biomaterials .
	manualset3
196278	1	416021	7	NULL	NULL	0	NULL	Ultrastructural analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural analysis of specific heart granules in the left atrial myocardium of the rat shows that the so-called A and B types are not different populations but represent varying planes of section through a uniform set of organelles .
	manualset3
196279	2	416021	7	NULL	NULL	NULL	NULL	specific heart granules	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ultrastructural analysis of specific heart granules in the left atrial myocardium of the rat shows that the so-called A and B types are not different populations but represent varying planes of section through a uniform set of organelles .
	manualset3
196280	3	416021	7	NULL	NULL	0	NULL	left atrial myocardium 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural analysis of specific heart granules in the left atrial myocardium of the rat shows that the so-called A and B types are not different populations but represent varying planes of section through a uniform set of organelles .
	manualset3
196281	4	416021	7	NULL	NULL	0	NULL	rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural analysis of specific heart granules in the left atrial myocardium of the rat shows that the so-called A and B types are not different populations but represent varying planes of section through a uniform set of organelles .
	manualset3
196282	5	416021	7	NULL	NULL	0	NULL	 A types	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural analysis of specific heart granules in the left atrial myocardium of the rat shows that the so-called A and B types are not different populations but represent varying planes of section through a uniform set of organelles .
	manualset3
196283	6	416021	7	NULL	NULL	0	NULL	B types	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural analysis of specific heart granules in the left atrial myocardium of the rat shows that the so-called A and B types are not different populations but represent varying planes of section through a uniform set of organelles .
	manualset3
196284	7	416021	7	NULL	NULL	0	NULL	 populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural analysis of specific heart granules in the left atrial myocardium of the rat shows that the so-called A and B types are not different populations but represent varying planes of section through a uniform set of organelles .
	manualset3
196285	8	416021	7	NULL	NULL	0	NULL	varying planes	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural analysis of specific heart granules in the left atrial myocardium of the rat shows that the so-called A and B types are not different populations but represent varying planes of section through a uniform set of organelles .
	manualset3
196286	9	416021	7	NULL	NULL	0	NULL	section	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural analysis of specific heart granules in the left atrial myocardium of the rat shows that the so-called A and B types are not different populations but represent varying planes of section through a uniform set of organelles .
	manualset3
196287	10	416021	7	NULL	NULL	0	NULL	uniform set 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural analysis of specific heart granules in the left atrial myocardium of the rat shows that the so-called A and B types are not different populations but represent varying planes of section through a uniform set of organelles .
	manualset3
196288	11	416021	7	NULL	NULL	0	NULL	organelles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural analysis of specific heart granules in the left atrial myocardium of the rat shows that the so-called A and B types are not different populations but represent varying planes of section through a uniform set of organelles .
	manualset3
196289	1	416022	7	NULL	NULL	0	NULL	Ultrastructural behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural behavior of human immunodeficiency virus ( HIV ) in multinucleated giant cells in the brain of a Japanese hemophiliac presenting AIDS encephalopathy .
	manualset3
196290	2	416022	7	NULL	NULL	0	NULL	human immunodeficiency virus ( HIV )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural behavior of human immunodeficiency virus ( HIV ) in multinucleated giant cells in the brain of a Japanese hemophiliac presenting AIDS encephalopathy .
	manualset3
196291	3	416022	7	NULL	NULL	0	NULL	multinucleated giant cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural behavior of human immunodeficiency virus ( HIV ) in multinucleated giant cells in the brain of a Japanese hemophiliac presenting AIDS encephalopathy .
	manualset3
196292	4	416022	7	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural behavior of human immunodeficiency virus ( HIV ) in multinucleated giant cells in the brain of a Japanese hemophiliac presenting AIDS encephalopathy .
	manualset3
196293	5	416022	7	NULL	NULL	0	NULL	Japanese hemophiliac	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural behavior of human immunodeficiency virus ( HIV ) in multinucleated giant cells in the brain of a Japanese hemophiliac presenting AIDS encephalopathy .
	manualset3
196294	6	416022	7	NULL	NULL	0	NULL	AIDS encephalopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural behavior of human immunodeficiency virus ( HIV ) in multinucleated giant cells in the brain of a Japanese hemophiliac presenting AIDS encephalopathy .
	manualset3
196295	1	416023	7	NULL	NULL	0	NULL	Ultrastructural changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural changes of endothelial cells of the mesenteric microcirculatory bed were morphometrically and statistically examined on a total of 32 male R-rats 15 , 30 , 60 , and 120 min after a traumatic-haemorrhagic shock ( THS ) .
	manualset3
196296	2	416023	7	NULL	NULL	0	NULL	endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural changes of endothelial cells of the mesenteric microcirculatory bed were morphometrically and statistically examined on a total of 32 male R-rats 15 , 30 , 60 , and 120 min after a traumatic-haemorrhagic shock ( THS ) .
	manualset3
196297	3	416023	7	NULL	NULL	0	NULL	mesenteric microcirculatory bed 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural changes of endothelial cells of the mesenteric microcirculatory bed were morphometrically and statistically examined on a total of 32 male R-rats 15 , 30 , 60 , and 120 min after a traumatic-haemorrhagic shock ( THS ) .
	manualset3
196298	4	416023	7	NULL	NULL	0	NULL	total	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural changes of endothelial cells of the mesenteric microcirculatory bed were morphometrically and statistically examined on a total of 32 male R-rats 15 , 30 , 60 , and 120 min after a traumatic-haemorrhagic shock ( THS ) .
	manualset3
196299	5	416023	7	NULL	NULL	0	NULL	32 male R-rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural changes of endothelial cells of the mesenteric microcirculatory bed were morphometrically and statistically examined on a total of 32 male R-rats 15 , 30 , 60 , and 120 min after a traumatic-haemorrhagic shock ( THS ) .
	manualset3
196300	6	416023	7	NULL	NULL	0	NULL	15 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural changes of endothelial cells of the mesenteric microcirculatory bed were morphometrically and statistically examined on a total of 32 male R-rats 15 , 30 , 60 , and 120 min after a traumatic-haemorrhagic shock ( THS ) .
	manualset3
196301	7	416023	7	NULL	NULL	0	NULL	30 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural changes of endothelial cells of the mesenteric microcirculatory bed were morphometrically and statistically examined on a total of 32 male R-rats 15 , 30 , 60 , and 120 min after a traumatic-haemorrhagic shock ( THS ) .
	manualset3
196302	8	416023	7	NULL	NULL	0	NULL	60 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural changes of endothelial cells of the mesenteric microcirculatory bed were morphometrically and statistically examined on a total of 32 male R-rats 15 , 30 , 60 , and 120 min after a traumatic-haemorrhagic shock ( THS ) .
	manualset3
196303	9	416023	7	NULL	NULL	0	NULL	120 min 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural changes of endothelial cells of the mesenteric microcirculatory bed were morphometrically and statistically examined on a total of 32 male R-rats 15 , 30 , 60 , and 120 min after a traumatic-haemorrhagic shock ( THS ) .
	manualset3
196304	10	416023	7	NULL	NULL	0	NULL	traumatic-haemorrhagic shock ( THS )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural changes of endothelial cells of the mesenteric microcirculatory bed were morphometrically and statistically examined on a total of 32 male R-rats 15 , 30 , 60 , and 120 min after a traumatic-haemorrhagic shock ( THS ) .
	manualset3
196305	1	416024	7	NULL	NULL	0	NULL	systemic work-up	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After systemic work-up for staging , we diagnosed the patient with multiple lymph node metastasis of the seminoma , and administered three cycles of bleomycin , etoposide , and cisplatin ( BEP ) therapy .
	manualset3
196306	2	416024	7	NULL	NULL	0	NULL	staging	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After systemic work-up for staging , we diagnosed the patient with multiple lymph node metastasis of the seminoma , and administered three cycles of bleomycin , etoposide , and cisplatin ( BEP ) therapy .
	manualset3
196307	3	416024	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	After systemic work-up for staging , we diagnosed the patient with multiple lymph node metastasis of the seminoma , and administered three cycles of bleomycin , etoposide , and cisplatin ( BEP ) therapy .
	manualset3
196308	4	416024	7	NULL	NULL	0	NULL	multiple lymph node metastasis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	After systemic work-up for staging , we diagnosed the patient with multiple lymph node metastasis of the seminoma , and administered three cycles of bleomycin , etoposide , and cisplatin ( BEP ) therapy .
	manualset3
196309	5	416024	7	NULL	NULL	0	NULL	seminoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	After systemic work-up for staging , we diagnosed the patient with multiple lymph node metastasis of the seminoma , and administered three cycles of bleomycin , etoposide , and cisplatin ( BEP ) therapy .
	manualset3
196310	6	416024	7	NULL	NULL	0	NULL	 three cycles	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After systemic work-up for staging , we diagnosed the patient with multiple lymph node metastasis of the seminoma , and administered three cycles of bleomycin , etoposide , and cisplatin ( BEP ) therapy .
	manualset3
196311	7	416024	7	NULL	NULL	0	NULL	bleomycin therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After systemic work-up for staging , we diagnosed the patient with multiple lymph node metastasis of the seminoma , and administered three cycles of bleomycin , etoposide , and cisplatin ( BEP ) therapy .
	manualset3
196312	8	416024	7	NULL	NULL	0	NULL	etoposide therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After systemic work-up for staging , we diagnosed the patient with multiple lymph node metastasis of the seminoma , and administered three cycles of bleomycin , etoposide , and cisplatin ( BEP ) therapy .
	manualset3
196313	9	416024	7	NULL	NULL	0	NULL	cisplatin therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After systemic work-up for staging , we diagnosed the patient with multiple lymph node metastasis of the seminoma , and administered three cycles of bleomycin , etoposide , and cisplatin ( BEP ) therapy .
	manualset3
196314	10	416024	7	NULL	NULL	0	NULL	BEP  therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After systemic work-up for staging , we diagnosed the patient with multiple lymph node metastasis of the seminoma , and administered three cycles of bleomycin , etoposide , and cisplatin ( BEP ) therapy .
	manualset3
196315	1	416025	7	NULL	NULL	0	NULL	Ultrastructural localisation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural localisation of Muc-1 on the plasma membrane of uterine epithelial cells .
	manualset3
196316	2	416025	7	NULL	NULL	0	NULL	Muc-1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural localisation of Muc-1 on the plasma membrane of uterine epithelial cells .
	manualset3
196317	3	416025	7	NULL	NULL	0	NULL	plasma membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural localisation of Muc-1 on the plasma membrane of uterine epithelial cells .
	manualset3
196318	4	416025	7	NULL	NULL	0	NULL	uterine epithelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural localisation of Muc-1 on the plasma membrane of uterine epithelial cells .
	manualset3
196319	1	416026	7	NULL	NULL	0	NULL	colocalization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructurally , a colocalization between beta-catenin and nuclear heterochromatin was demonstrated .
	manualset3
196320	2	416026	7	NULL	NULL	0	NULL	beta-catenin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructurally , a colocalization between beta-catenin and nuclear heterochromatin was demonstrated .
	manualset3
196321	3	416026	7	NULL	NULL	0	NULL	 nuclear heterochromatin	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructurally , a colocalization between beta-catenin and nuclear heterochromatin was demonstrated .
	manualset3
196322	1	416027	7	NULL	NULL	0	NULL	filamentous material	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructurally , the filamentous material was seen within the mesangial granulomas and also in a subendothelial location , suggesting derivation from the circulation with subsequent transport across the basement membrane and accumulation in the mesangium , where a granulomatous reaction was elicited .
	manualset3
196323	2	416027	7	NULL	NULL	0	NULL	mesangial granulomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructurally , the filamentous material was seen within the mesangial granulomas and also in a subendothelial location , suggesting derivation from the circulation with subsequent transport across the basement membrane and accumulation in the mesangium , where a granulomatous reaction was elicited .
	manualset3
196324	3	416027	7	NULL	NULL	0	NULL	subendothelial location	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructurally , the filamentous material was seen within the mesangial granulomas and also in a subendothelial location , suggesting derivation from the circulation with subsequent transport across the basement membrane and accumulation in the mesangium , where a granulomatous reaction was elicited .
	manualset3
196325	4	416027	7	NULL	NULL	0	NULL	derivation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructurally , the filamentous material was seen within the mesangial granulomas and also in a subendothelial location , suggesting derivation from the circulation with subsequent transport across the basement membrane and accumulation in the mesangium , where a granulomatous reaction was elicited .
	manualset3
196326	5	416027	7	NULL	NULL	0	NULL	 circulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructurally , the filamentous material was seen within the mesangial granulomas and also in a subendothelial location , suggesting derivation from the circulation with subsequent transport across the basement membrane and accumulation in the mesangium , where a granulomatous reaction was elicited .
	manualset3
196327	6	416027	7	NULL	NULL	0	NULL	transport	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructurally , the filamentous material was seen within the mesangial granulomas and also in a subendothelial location , suggesting derivation from the circulation with subsequent transport across the basement membrane and accumulation in the mesangium , where a granulomatous reaction was elicited .
	manualset3
196328	7	416027	7	NULL	NULL	0	NULL	basement membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructurally , the filamentous material was seen within the mesangial granulomas and also in a subendothelial location , suggesting derivation from the circulation with subsequent transport across the basement membrane and accumulation in the mesangium , where a granulomatous reaction was elicited .
	manualset3
196329	8	416027	7	NULL	NULL	0	NULL	accumulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructurally , the filamentous material was seen within the mesangial granulomas and also in a subendothelial location , suggesting derivation from the circulation with subsequent transport across the basement membrane and accumulation in the mesangium , where a granulomatous reaction was elicited .
	manualset3
196330	9	416027	7	NULL	NULL	0	NULL	mesangium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructurally , the filamentous material was seen within the mesangial granulomas and also in a subendothelial location , suggesting derivation from the circulation with subsequent transport across the basement membrane and accumulation in the mesangium , where a granulomatous reaction was elicited .
	manualset3
196331	10	416027	7	NULL	NULL	0	NULL	granulomatous reaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructurally , the filamentous material was seen within the mesangial granulomas and also in a subendothelial location , suggesting derivation from the circulation with subsequent transport across the basement membrane and accumulation in the mesangium , where a granulomatous reaction was elicited .
	manualset3
196332	1	416028	7	NULL	NULL	0	NULL	Ultrastructure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructure of Purkinje cell perikarya and their dendritic processes in the rat cerebellar cortex in experimental encephalopathy induced by chronic application of valproate .
	manualset3
196333	2	416028	7	NULL	NULL	0	NULL	 Purkinje cell perikarya	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructure of Purkinje cell perikarya and their dendritic processes in the rat cerebellar cortex in experimental encephalopathy induced by chronic application of valproate .
	manualset3
196334	3	416028	7	NULL	NULL	0	NULL	dendritic processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructure of Purkinje cell perikarya and their dendritic processes in the rat cerebellar cortex in experimental encephalopathy induced by chronic application of valproate .
	manualset3
196335	4	416028	7	NULL	NULL	0	NULL	rat cerebellar cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructure of Purkinje cell perikarya and their dendritic processes in the rat cerebellar cortex in experimental encephalopathy induced by chronic application of valproate .
	manualset3
196336	5	416028	7	NULL	NULL	0	NULL	experimental encephalopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructure of Purkinje cell perikarya and their dendritic processes in the rat cerebellar cortex in experimental encephalopathy induced by chronic application of valproate .
	manualset3
196337	6	416028	7	NULL	NULL	0	NULL	chronic application	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructure of Purkinje cell perikarya and their dendritic processes in the rat cerebellar cortex in experimental encephalopathy induced by chronic application of valproate .
	manualset3
196338	7	416028	7	NULL	NULL	0	NULL	valproate	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructure of Purkinje cell perikarya and their dendritic processes in the rat cerebellar cortex in experimental encephalopathy induced by chronic application of valproate .
	manualset3
196339	1	416029	7	NULL	NULL	0	NULL	Ultraviolet-induced reversion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultraviolet-induced reversion of cyc1 alleles in radiation-sensitive strains of yeast .
	manualset3
196340	2	416029	7	NULL	NULL	NULL	NULL	cyc1 alleles	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ultraviolet-induced reversion of cyc1 alleles in radiation-sensitive strains of yeast .
	manualset3
196341	3	416029	7	NULL	NULL	0	NULL	radiation-sensitive strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultraviolet-induced reversion of cyc1 alleles in radiation-sensitive strains of yeast .
	manualset3
196342	4	416029	7	NULL	NULL	0	NULL	 yeast	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultraviolet-induced reversion of cyc1 alleles in radiation-sensitive strains of yeast .
	manualset3
196343	1	416030	7	NULL	NULL	0	NULL	Ultraviolet analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultraviolet analysis of donated corneas : a portable prototype .
	manualset3
196344	2	416030	7	NULL	NULL	0	NULL	donated corneas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultraviolet analysis of donated corneas : a portable prototype .
	manualset3
196345	3	416030	7	NULL	NULL	0	NULL	portable prototype	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultraviolet analysis of donated corneas : a portable prototype .
	manualset3
196348	1	416031	7	NULL	NULL	0	NULL	Unassisted walking velocity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Unassisted walking velocity increased 22 % , stride length increased 13 % , and cadence increased 7 % .
	manualset3
196349	2	416031	7	NULL	NULL	0	NULL	22 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Unassisted walking velocity increased 22 % , stride length increased 13 % , and cadence increased 7 % .
	manualset3
196350	3	416031	7	NULL	NULL	0	NULL	stride length	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Unassisted walking velocity increased 22 % , stride length increased 13 % , and cadence increased 7 % .
	manualset3
196351	4	416031	7	NULL	NULL	0	NULL	13 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Unassisted walking velocity increased 22 % , stride length increased 13 % , and cadence increased 7 % .
	manualset3
196352	5	416031	7	NULL	NULL	0	NULL	cadence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Unassisted walking velocity increased 22 % , stride length increased 13 % , and cadence increased 7 % .
	manualset3
196353	6	416031	7	NULL	NULL	0	NULL	7 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Unassisted walking velocity increased 22 % , stride length increased 13 % , and cadence increased 7 % .
	manualset3
196354	1	416032	7	NULL	NULL	0	NULL	 consideration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Uncertainty is an important consideration for both developers and users of environmental simulation models .
	manualset3
196355	2	416032	7	NULL	NULL	0	NULL	developers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Uncertainty is an important consideration for both developers and users of environmental simulation models .
	manualset3
196356	3	416032	7	NULL	NULL	0	NULL	users 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Uncertainty is an important consideration for both developers and users of environmental simulation models .
	manualset3
196357	4	416032	7	NULL	NULL	0	NULL	environmental simulation models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Uncertainty is an important consideration for both developers and users of environmental simulation models .
	manualset3
196358	1	416033	7	NULL	NULL	0	NULL	Uncoupling results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Uncoupling results from breakdown of X approximately acyl , but sufficient X approximately acyl is maintained to serve as a source of activated fatty acid .
	manualset3
196359	2	416033	7	NULL	NULL	0	NULL	breakdown	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Uncoupling results from breakdown of X approximately acyl , but sufficient X approximately acyl is maintained to serve as a source of activated fatty acid .
	manualset3
196360	3	416033	7	NULL	NULL	0	NULL	X	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Uncoupling results from breakdown of X approximately acyl , but sufficient X approximately acyl is maintained to serve as a source of activated fatty acid .
	manualset3
196361	4	416033	7	NULL	NULL	0	NULL	acyl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Uncoupling results from breakdown of X approximately acyl , but sufficient X approximately acyl is maintained to serve as a source of activated fatty acid .
	manualset3
196362	5	416033	7	NULL	NULL	0	NULL	X	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Uncoupling results from breakdown of X approximately acyl , but sufficient X approximately acyl is maintained to serve as a source of activated fatty acid .
	manualset3
196363	6	416033	7	NULL	NULL	0	NULL	acyl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Uncoupling results from breakdown of X approximately acyl , but sufficient X approximately acyl is maintained to serve as a source of activated fatty acid .
	manualset3
196364	7	416033	7	NULL	NULL	0	NULL	source	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Uncoupling results from breakdown of X approximately acyl , but sufficient X approximately acyl is maintained to serve as a source of activated fatty acid .
	manualset3
196365	8	416033	7	NULL	NULL	0	NULL	activated fatty acid	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Uncoupling results from breakdown of X approximately acyl , but sufficient X approximately acyl is maintained to serve as a source of activated fatty acid .
	manualset3
196366	1	416034	7	NULL	NULL	0	NULL	conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Under all conditions that we have used for electron microscopy , including the absence of nucleotide , some rings exist as trimers of dimers , showing that the symmetry of the DnaB hexamer can be broken prior to nucleotide binding .
	manualset3
196367	2	416034	7	NULL	NULL	0	NULL	electron microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Under all conditions that we have used for electron microscopy , including the absence of nucleotide , some rings exist as trimers of dimers , showing that the symmetry of the DnaB hexamer can be broken prior to nucleotide binding .
	manualset3
196368	3	416034	7	NULL	NULL	0	NULL	nucleotide	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Under all conditions that we have used for electron microscopy , including the absence of nucleotide , some rings exist as trimers of dimers , showing that the symmetry of the DnaB hexamer can be broken prior to nucleotide binding .
	manualset3
196369	4	416034	7	NULL	NULL	0	NULL	rings	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Under all conditions that we have used for electron microscopy , including the absence of nucleotide , some rings exist as trimers of dimers , showing that the symmetry of the DnaB hexamer can be broken prior to nucleotide binding .
	manualset3
196370	5	416034	7	NULL	NULL	0	NULL	trimers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Under all conditions that we have used for electron microscopy , including the absence of nucleotide , some rings exist as trimers of dimers , showing that the symmetry of the DnaB hexamer can be broken prior to nucleotide binding .
	manualset3
196371	6	416034	7	NULL	NULL	0	NULL	dimers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Under all conditions that we have used for electron microscopy , including the absence of nucleotide , some rings exist as trimers of dimers , showing that the symmetry of the DnaB hexamer can be broken prior to nucleotide binding .
	manualset3
196372	7	416034	7	NULL	NULL	0	NULL	symmetry	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Under all conditions that we have used for electron microscopy , including the absence of nucleotide , some rings exist as trimers of dimers , showing that the symmetry of the DnaB hexamer can be broken prior to nucleotide binding .
	manualset3
196373	8	416034	7	NULL	NULL	0	NULL	DnaB hexamer 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Under all conditions that we have used for electron microscopy , including the absence of nucleotide , some rings exist as trimers of dimers , showing that the symmetry of the DnaB hexamer can be broken prior to nucleotide binding .
	manualset3
196374	9	416034	7	NULL	NULL	0	NULL	nucleotide binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Under all conditions that we have used for electron microscopy , including the absence of nucleotide , some rings exist as trimers of dimers , showing that the symmetry of the DnaB hexamer can be broken prior to nucleotide binding .
	manualset3
196375	1	416035	7	NULL	NULL	0	NULL	creatine supplement	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	After taking the creatine supplement , task-evoked increase of cerebral oxygenated hemoglobin in the brains of subjects measured by near infrared spectroscopy was significantly reduced , which is compatible with increased oxygen utilization in the brain .
	manualset3
196376	2	416035	7	NULL	NULL	0	NULL	task-evoked increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After taking the creatine supplement , task-evoked increase of cerebral oxygenated hemoglobin in the brains of subjects measured by near infrared spectroscopy was significantly reduced , which is compatible with increased oxygen utilization in the brain .
	manualset3
196377	3	416035	7	NULL	NULL	NULL	NULL	cerebral oxygenated hemoglobin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After taking the creatine supplement , task-evoked increase of cerebral oxygenated hemoglobin in the brains of subjects measured by near infrared spectroscopy was significantly reduced , which is compatible with increased oxygen utilization in the brain .
	manualset3
196378	4	416035	7	NULL	NULL	0	NULL	brains	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After taking the creatine supplement , task-evoked increase of cerebral oxygenated hemoglobin in the brains of subjects measured by near infrared spectroscopy was significantly reduced , which is compatible with increased oxygen utilization in the brain .
	manualset3
196379	5	416035	7	NULL	NULL	0	NULL	subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	After taking the creatine supplement , task-evoked increase of cerebral oxygenated hemoglobin in the brains of subjects measured by near infrared spectroscopy was significantly reduced , which is compatible with increased oxygen utilization in the brain .
	manualset3
196380	6	416035	7	NULL	NULL	0	NULL	near infrared spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After taking the creatine supplement , task-evoked increase of cerebral oxygenated hemoglobin in the brains of subjects measured by near infrared spectroscopy was significantly reduced , which is compatible with increased oxygen utilization in the brain .
	manualset3
196381	7	416035	7	NULL	NULL	0	NULL	oxygen utilization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After taking the creatine supplement , task-evoked increase of cerebral oxygenated hemoglobin in the brains of subjects measured by near infrared spectroscopy was significantly reduced , which is compatible with increased oxygen utilization in the brain .
	manualset3
196382	8	416035	7	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After taking the creatine supplement , task-evoked increase of cerebral oxygenated hemoglobin in the brains of subjects measured by near infrared spectroscopy was significantly reduced , which is compatible with increased oxygen utilization in the brain .
	manualset3
196383	1	416036	7	NULL	NULL	0	NULL	conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Under all conditions the conversion of cholesterol into pregnenolone is the ( hormonal regulated ) rate-determining step for steroidogenesis .
	manualset3
196384	2	416036	7	NULL	NULL	0	NULL	conversion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Under all conditions the conversion of cholesterol into pregnenolone is the ( hormonal regulated ) rate-determining step for steroidogenesis .
	manualset3
196385	3	416036	7	NULL	NULL	0	NULL	cholesterol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Under all conditions the conversion of cholesterol into pregnenolone is the ( hormonal regulated ) rate-determining step for steroidogenesis .
	manualset3
196386	4	416036	7	NULL	NULL	0	NULL	pregnenolone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Under all conditions the conversion of cholesterol into pregnenolone is the ( hormonal regulated ) rate-determining step for steroidogenesis .
	manualset3
196387	5	416036	7	NULL	NULL	0	NULL	rate-determining step	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Under all conditions the conversion of cholesterol into pregnenolone is the ( hormonal regulated ) rate-determining step for steroidogenesis .
	manualset3
196388	6	416036	7	NULL	NULL	0	NULL	steroidogenesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Under all conditions the conversion of cholesterol into pregnenolone is the ( hormonal regulated ) rate-determining step for steroidogenesis .
	manualset3
196389	1	416037	7	NULL	NULL	0	NULL	anaesthesia	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Under anaesthesia , five sheep fetuses were instrumented with catheters and a Transonic probe around an umbilical artery , inside the fetal abdomen , at 0.8 of gestation .
	manualset3
196390	2	416037	7	NULL	NULL	0	NULL	five sheep fetuses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Under anaesthesia , five sheep fetuses were instrumented with catheters and a Transonic probe around an umbilical artery , inside the fetal abdomen , at 0.8 of gestation .
	manualset3
196391	3	416037	7	NULL	NULL	0	NULL	catheters	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Under anaesthesia , five sheep fetuses were instrumented with catheters and a Transonic probe around an umbilical artery , inside the fetal abdomen , at 0.8 of gestation .
	manualset3
196392	4	416037	7	NULL	NULL	0	NULL	Transonic probe	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Under anaesthesia , five sheep fetuses were instrumented with catheters and a Transonic probe around an umbilical artery , inside the fetal abdomen , at 0.8 of gestation .
	manualset3
196393	5	416037	7	NULL	NULL	0	NULL	umbilical artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Under anaesthesia , five sheep fetuses were instrumented with catheters and a Transonic probe around an umbilical artery , inside the fetal abdomen , at 0.8 of gestation .
	manualset3
196394	6	416037	7	NULL	NULL	0	NULL	fetal abdomen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Under anaesthesia , five sheep fetuses were instrumented with catheters and a Transonic probe around an umbilical artery , inside the fetal abdomen , at 0.8 of gestation .
	manualset3
196395	7	416037	7	NULL	NULL	0	NULL	0.8	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Under anaesthesia , five sheep fetuses were instrumented with catheters and a Transonic probe around an umbilical artery , inside the fetal abdomen , at 0.8 of gestation .
	manualset3
196396	8	416037	7	NULL	NULL	0	NULL	 gestation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Under anaesthesia , five sheep fetuses were instrumented with catheters and a Transonic probe around an umbilical artery , inside the fetal abdomen , at 0.8 of gestation .
	manualset3
196397	1	416038	7	NULL	NULL	NULL	NULL	antibiotic treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Under antibiotic treatment with clarithromycin and doxycycline the fever and the hyperbilirubinemia decreased .
	manualset3
196398	2	416038	7	NULL	NULL	0	NULL	clarithromycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Under antibiotic treatment with clarithromycin and doxycycline the fever and the hyperbilirubinemia decreased .
	manualset3
196399	3	416038	7	NULL	NULL	0	NULL	doxycycline	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Under antibiotic treatment with clarithromycin and doxycycline the fever and the hyperbilirubinemia decreased .
	manualset3
196400	4	416038	7	NULL	NULL	0	NULL	fever	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Under antibiotic treatment with clarithromycin and doxycycline the fever and the hyperbilirubinemia decreased .
	manualset3
196401	5	416038	7	NULL	NULL	0	NULL	hyperbilirubinemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Under antibiotic treatment with clarithromycin and doxycycline the fever and the hyperbilirubinemia decreased .
	manualset3
196402	1	416039	7	NULL	NULL	0	NULL	basal conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Under basal conditions this metabolite appears to be effectively detoxified , but increased CYP2E1 activity and/or decreased aldehyde dehydrogenase activity promotes accumulation of metabolite , and therefore increases glutathione depletion and toxicity .
	manualset3
196403	2	416039	7	NULL	NULL	0	NULL	metabolite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Under basal conditions this metabolite appears to be effectively detoxified , but increased CYP2E1 activity and/or decreased aldehyde dehydrogenase activity promotes accumulation of metabolite , and therefore increases glutathione depletion and toxicity .
	manualset3
196404	3	416039	7	NULL	NULL	0	NULL	increased CYP2E1 activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Under basal conditions this metabolite appears to be effectively detoxified , but increased CYP2E1 activity and/or decreased aldehyde dehydrogenase activity promotes accumulation of metabolite , and therefore increases glutathione depletion and toxicity .
	manualset3
196405	4	416039	7	NULL	NULL	0	NULL	decreased aldehyde dehydrogenase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Under basal conditions this metabolite appears to be effectively detoxified , but increased CYP2E1 activity and/or decreased aldehyde dehydrogenase activity promotes accumulation of metabolite , and therefore increases glutathione depletion and toxicity .
	manualset3
196406	5	416039	7	NULL	NULL	0	NULL	accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Under basal conditions this metabolite appears to be effectively detoxified , but increased CYP2E1 activity and/or decreased aldehyde dehydrogenase activity promotes accumulation of metabolite , and therefore increases glutathione depletion and toxicity .
	manualset3
196407	6	416039	7	NULL	NULL	0	NULL	metabolite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Under basal conditions this metabolite appears to be effectively detoxified , but increased CYP2E1 activity and/or decreased aldehyde dehydrogenase activity promotes accumulation of metabolite , and therefore increases glutathione depletion and toxicity .
	manualset3
196408	7	416039	7	NULL	NULL	0	NULL	 glutathione depletion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Under basal conditions this metabolite appears to be effectively detoxified , but increased CYP2E1 activity and/or decreased aldehyde dehydrogenase activity promotes accumulation of metabolite , and therefore increases glutathione depletion and toxicity .
	manualset3
196409	8	416039	7	NULL	NULL	NULL	NULL	toxicity 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Under basal conditions this metabolite appears to be effectively detoxified , but increased CYP2E1 activity and/or decreased aldehyde dehydrogenase activity promotes accumulation of metabolite , and therefore increases glutathione depletion and toxicity .
	manualset3
196410	1	416040	7	NULL	NULL	0	NULL	 coculture conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Under coculture conditions , the peripheral processes invade the vibrissa pad explants and form a characteristic circumfollicular pattern .
	manualset3
196411	2	416040	7	NULL	NULL	0	NULL	peripheral processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Under coculture conditions , the peripheral processes invade the vibrissa pad explants and form a characteristic circumfollicular pattern .
	manualset3
196412	3	416040	7	NULL	NULL	0	NULL	vibrissa pad explants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Under coculture conditions , the peripheral processes invade the vibrissa pad explants and form a characteristic circumfollicular pattern .
	manualset3
196413	4	416040	7	NULL	NULL	0	NULL	circumfollicular pattern	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Under coculture conditions , the peripheral processes invade the vibrissa pad explants and form a characteristic circumfollicular pattern .
	manualset3
196414	1	416041	7	NULL	NULL	0	NULL	condition	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Under condition ( a ) , administration of L-citrulline , L-carnitine , and L-acetylcarnitine improved the protective effect of 5FMOrn significantly , in an additive manner .
	manualset3
196415	2	416041	7	NULL	NULL	0	NULL	administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Under condition ( a ) , administration of L-citrulline , L-carnitine , and L-acetylcarnitine improved the protective effect of 5FMOrn significantly , in an additive manner .
	manualset3
196416	3	416041	7	NULL	NULL	0	NULL	L-citrulline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Under condition ( a ) , administration of L-citrulline , L-carnitine , and L-acetylcarnitine improved the protective effect of 5FMOrn significantly , in an additive manner .
	manualset3
196417	4	416041	7	NULL	NULL	0	NULL	L-carnitine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Under condition ( a ) , administration of L-citrulline , L-carnitine , and L-acetylcarnitine improved the protective effect of 5FMOrn significantly , in an additive manner .
	manualset3
196418	5	416041	7	NULL	NULL	0	NULL	L-acetylcarnitine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Under condition ( a ) , administration of L-citrulline , L-carnitine , and L-acetylcarnitine improved the protective effect of 5FMOrn significantly , in an additive manner .
	manualset3
196419	6	416041	7	NULL	NULL	0	NULL	protective effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Under condition ( a ) , administration of L-citrulline , L-carnitine , and L-acetylcarnitine improved the protective effect of 5FMOrn significantly , in an additive manner .
	manualset3
196420	7	416041	7	NULL	NULL	0	NULL	 5FMOrn	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Under condition ( a ) , administration of L-citrulline , L-carnitine , and L-acetylcarnitine improved the protective effect of 5FMOrn significantly , in an additive manner .
	manualset3
196421	8	416041	7	NULL	NULL	0	NULL	additive manner	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Under condition ( a ) , administration of L-citrulline , L-carnitine , and L-acetylcarnitine improved the protective effect of 5FMOrn significantly , in an additive manner .
	manualset3
196422	1	416042	7	NULL	NULL	0	NULL	conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Under conditions of an intensified immune response , many eukaryotic cells adapt by replacing standard 20 S proteasomes with immuno-proteasomes and/or generating the proteasome activator complex , PA28 .
	manualset3
196423	2	416042	7	NULL	NULL	0	NULL	 intensified immune response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Under conditions of an intensified immune response , many eukaryotic cells adapt by replacing standard 20 S proteasomes with immuno-proteasomes and/or generating the proteasome activator complex , PA28 .
	manualset3
196424	3	416042	7	NULL	NULL	0	NULL	eukaryotic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Under conditions of an intensified immune response , many eukaryotic cells adapt by replacing standard 20 S proteasomes with immuno-proteasomes and/or generating the proteasome activator complex , PA28 .
	manualset3
196425	4	416042	7	NULL	NULL	0	NULL	standard 20 S proteasomes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Under conditions of an intensified immune response , many eukaryotic cells adapt by replacing standard 20 S proteasomes with immuno-proteasomes and/or generating the proteasome activator complex , PA28 .
	manualset3
196426	5	416042	7	NULL	NULL	0	NULL	immuno-proteasomes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Under conditions of an intensified immune response , many eukaryotic cells adapt by replacing standard 20 S proteasomes with immuno-proteasomes and/or generating the proteasome activator complex , PA28 .
	manualset3
196427	6	416042	7	NULL	NULL	0	NULL	proteasome activator complex , PA28	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Under conditions of an intensified immune response , many eukaryotic cells adapt by replacing standard 20 S proteasomes with immuno-proteasomes and/or generating the proteasome activator complex , PA28 .
	manualset3
196428	1	416043	7	NULL	NULL	0	NULL	dietary condition	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Under each dietary condition , subjects were infused postabsorptively with L - ( 1-13C ) leucine , L - ( 15N ) alanine , and L - ( 3 , 3 , 3-2H3 ) alanine to measure leucine and alanine kinetics .
	manualset3
196429	2	416043	7	NULL	NULL	0	NULL	subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Under each dietary condition , subjects were infused postabsorptively with L - ( 1-13C ) leucine , L - ( 15N ) alanine , and L - ( 3 , 3 , 3-2H3 ) alanine to measure leucine and alanine kinetics .
	manualset3
196430	3	416043	7	NULL	NULL	0	NULL	L - ( 1-13C ) leucine 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Under each dietary condition , subjects were infused postabsorptively with L - ( 1-13C ) leucine , L - ( 15N ) alanine , and L - ( 3 , 3 , 3-2H3 ) alanine to measure leucine and alanine kinetics .
	manualset3
196431	4	416043	7	NULL	NULL	0	NULL	L - ( 15N ) alanine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Under each dietary condition , subjects were infused postabsorptively with L - ( 1-13C ) leucine , L - ( 15N ) alanine , and L - ( 3 , 3 , 3-2H3 ) alanine to measure leucine and alanine kinetics .
	manualset3
196432	5	416043	7	NULL	NULL	0	NULL	L - ( 3 , 3 , 3-2H3 ) alanine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Under each dietary condition , subjects were infused postabsorptively with L - ( 1-13C ) leucine , L - ( 15N ) alanine , and L - ( 3 , 3 , 3-2H3 ) alanine to measure leucine and alanine kinetics .
	manualset3
196433	6	416043	7	NULL	NULL	0	NULL	 leucine kinetics	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Under each dietary condition , subjects were infused postabsorptively with L - ( 1-13C ) leucine , L - ( 15N ) alanine , and L - ( 3 , 3 , 3-2H3 ) alanine to measure leucine and alanine kinetics .
	manualset3
196434	7	416043	7	NULL	NULL	0	NULL	alanine kinetics	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Under each dietary condition , subjects were infused postabsorptively with L - ( 1-13C ) leucine , L - ( 15N ) alanine , and L - ( 3 , 3 , 3-2H3 ) alanine to measure leucine and alanine kinetics .
	manualset3
196435	1	416044	7	NULL	NULL	0	NULL	electron microscopic observation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Under electron microscopic observation , the virus particles were found in the tissues of the central nervous system of the affected larval striped jack .
	manualset3
196436	2	416044	7	NULL	NULL	0	NULL	virus particles	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Under electron microscopic observation , the virus particles were found in the tissues of the central nervous system of the affected larval striped jack .
	manualset3
196437	3	416044	7	NULL	NULL	0	NULL	tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Under electron microscopic observation , the virus particles were found in the tissues of the central nervous system of the affected larval striped jack .
	manualset3
196438	4	416044	7	NULL	NULL	0	NULL	central nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Under electron microscopic observation , the virus particles were found in the tissues of the central nervous system of the affected larval striped jack .
	manualset3
196439	5	416044	7	NULL	NULL	0	NULL	larval striped jack	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Under electron microscopic observation , the virus particles were found in the tissues of the central nervous system of the affected larval striped jack .
	manualset3
196440	1	416045	7	NULL	NULL	NULL	NULL	 Women 's Health Initiative	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After the Women 's Health Initiative : Postmenopausal women 's experiences with discontinuing estrogen replacement therapy .
	manualset3
196441	2	416045	7	NULL	NULL	NULL	NULL	Postmenopausal women 's experiences	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After the Women 's Health Initiative : Postmenopausal women 's experiences with discontinuing estrogen replacement therapy .
	manualset3
196442	3	416045	7	NULL	NULL	0	NULL	 estrogen replacement therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After the Women 's Health Initiative : Postmenopausal women 's experiences with discontinuing estrogen replacement therapy .
	manualset3
196443	1	416046	7	NULL	NULL	0	NULL	GB99 + GB122	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Under most circumstances , GB99 + GB122 suppressed nematode reproduction more consistently than ASM compared to the untreated control .
	manualset3
196444	2	416046	7	NULL	NULL	0	NULL	 nematode reproduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Under most circumstances , GB99 + GB122 suppressed nematode reproduction more consistently than ASM compared to the untreated control .
	manualset3
196445	3	416046	7	NULL	NULL	0	NULL	ASM	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Under most circumstances , GB99 + GB122 suppressed nematode reproduction more consistently than ASM compared to the untreated control .
	manualset3
196446	4	416046	7	NULL	NULL	0	NULL	 untreated control	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Under most circumstances , GB99 + GB122 suppressed nematode reproduction more consistently than ASM compared to the untreated control .
	manualset3
196447	5	416046	7	NULL	NULL	0	NULL	circumstances	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Under most circumstances , GB99 + GB122 suppressed nematode reproduction more consistently than ASM compared to the untreated control .
	manualset3
196448	1	416047	7	NULL	NULL	0	NULL	novel stimulus conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Under novel ( but not familiar ) stimulus conditions haloperidol-treated rats showed an enhancement of spontaneous activity , similar to that observed in vehicle-treated animals , and exceeded their previous low rates of crossing and rearing responses .
	manualset3
196449	2	416047	7	NULL	NULL	0	NULL	haloperidol-treated rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Under novel ( but not familiar ) stimulus conditions haloperidol-treated rats showed an enhancement of spontaneous activity , similar to that observed in vehicle-treated animals , and exceeded their previous low rates of crossing and rearing responses .
	manualset3
196450	3	416047	7	NULL	NULL	0	NULL	enhancement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Under novel ( but not familiar ) stimulus conditions haloperidol-treated rats showed an enhancement of spontaneous activity , similar to that observed in vehicle-treated animals , and exceeded their previous low rates of crossing and rearing responses .
	manualset3
196451	4	416047	7	NULL	NULL	0	NULL	spontaneous activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Under novel ( but not familiar ) stimulus conditions haloperidol-treated rats showed an enhancement of spontaneous activity , similar to that observed in vehicle-treated animals , and exceeded their previous low rates of crossing and rearing responses .
	manualset3
196452	5	416047	7	NULL	NULL	0	NULL	 vehicle-treated animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Under novel ( but not familiar ) stimulus conditions haloperidol-treated rats showed an enhancement of spontaneous activity , similar to that observed in vehicle-treated animals , and exceeded their previous low rates of crossing and rearing responses .
	manualset3
196453	6	416047	7	NULL	NULL	0	NULL	low rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Under novel ( but not familiar ) stimulus conditions haloperidol-treated rats showed an enhancement of spontaneous activity , similar to that observed in vehicle-treated animals , and exceeded their previous low rates of crossing and rearing responses .
	manualset3
196454	7	416047	7	NULL	NULL	0	NULL	 crossing responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Under novel ( but not familiar ) stimulus conditions haloperidol-treated rats showed an enhancement of spontaneous activity , similar to that observed in vehicle-treated animals , and exceeded their previous low rates of crossing and rearing responses .
	manualset3
196455	8	416047	7	NULL	NULL	0	NULL	 rearing responses 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Under novel ( but not familiar ) stimulus conditions haloperidol-treated rats showed an enhancement of spontaneous activity , similar to that observed in vehicle-treated animals , and exceeded their previous low rates of crossing and rearing responses .
	manualset3
196456	1	416048	7	NULL	NULL	0	NULL	optimum conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Under optimum conditions ( phosphate buffer , pH 7.5 and 30C ) , the inhibition of AChE by malathion and chlorpyrifos was proportional to their concentrations in the range , 0.1-50nM and 1.5-40nM , respectively .
	manualset3
196457	2	416048	7	NULL	NULL	0	NULL	phosphate buffer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Under optimum conditions ( phosphate buffer , pH 7.5 and 30C ) , the inhibition of AChE by malathion and chlorpyrifos was proportional to their concentrations in the range , 0.1-50nM and 1.5-40nM , respectively .
	manualset3
196458	3	416048	7	NULL	NULL	0	NULL	pH 7.5	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Under optimum conditions ( phosphate buffer , pH 7.5 and 30C ) , the inhibition of AChE by malathion and chlorpyrifos was proportional to their concentrations in the range , 0.1-50nM and 1.5-40nM , respectively .
	manualset3
196459	4	416048	7	NULL	NULL	0	NULL	30C	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Under optimum conditions ( phosphate buffer , pH 7.5 and 30C ) , the inhibition of AChE by malathion and chlorpyrifos was proportional to their concentrations in the range , 0.1-50nM and 1.5-40nM , respectively .
	manualset3
196460	5	416048	7	NULL	NULL	0	NULL	 inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Under optimum conditions ( phosphate buffer , pH 7.5 and 30C ) , the inhibition of AChE by malathion and chlorpyrifos was proportional to their concentrations in the range , 0.1-50nM and 1.5-40nM , respectively .
	manualset3
196461	6	416048	7	NULL	NULL	0	NULL	 AChE	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Under optimum conditions ( phosphate buffer , pH 7.5 and 30C ) , the inhibition of AChE by malathion and chlorpyrifos was proportional to their concentrations in the range , 0.1-50nM and 1.5-40nM , respectively .
	manualset3
196462	7	416048	7	NULL	NULL	0	NULL	malathion	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Under optimum conditions ( phosphate buffer , pH 7.5 and 30C ) , the inhibition of AChE by malathion and chlorpyrifos was proportional to their concentrations in the range , 0.1-50nM and 1.5-40nM , respectively .
	manualset3
196463	8	416048	7	NULL	NULL	0	NULL	chlorpyrifos	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Under optimum conditions ( phosphate buffer , pH 7.5 and 30C ) , the inhibition of AChE by malathion and chlorpyrifos was proportional to their concentrations in the range , 0.1-50nM and 1.5-40nM , respectively .
	manualset3
196464	9	416048	7	NULL	NULL	0	NULL	concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Under optimum conditions ( phosphate buffer , pH 7.5 and 30C ) , the inhibition of AChE by malathion and chlorpyrifos was proportional to their concentrations in the range , 0.1-50nM and 1.5-40nM , respectively .
	manualset3
196465	10	416048	7	NULL	NULL	0	NULL	range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Under optimum conditions ( phosphate buffer , pH 7.5 and 30C ) , the inhibition of AChE by malathion and chlorpyrifos was proportional to their concentrations in the range , 0.1-50nM and 1.5-40nM , respectively .
	manualset3
196466	11	416048	7	NULL	NULL	0	NULL	0.1-50nM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Under optimum conditions ( phosphate buffer , pH 7.5 and 30C ) , the inhibition of AChE by malathion and chlorpyrifos was proportional to their concentrations in the range , 0.1-50nM and 1.5-40nM , respectively .
	manualset3
196467	12	416048	7	NULL	NULL	0	NULL	1.5-40nM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Under optimum conditions ( phosphate buffer , pH 7.5 and 30C ) , the inhibition of AChE by malathion and chlorpyrifos was proportional to their concentrations in the range , 0.1-50nM and 1.5-40nM , respectively .
	manualset3
196468	1	416049	7	NULL	NULL	0	NULL	optimum conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Under optimum conditions , ascertained by evaluating various electrochemical parameters , the accuracy and precision ( 95 % ts ) were found to be + / - 0.3 % .
	manualset3
196469	2	416049	7	NULL	NULL	0	NULL	electrochemical parameters	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Under optimum conditions , ascertained by evaluating various electrochemical parameters , the accuracy and precision ( 95 % ts ) were found to be + / - 0.3 % .
	manualset3
196470	3	416049	7	NULL	NULL	0	NULL	accuracy	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Under optimum conditions , ascertained by evaluating various electrochemical parameters , the accuracy and precision ( 95 % ts ) were found to be + / - 0.3 % .
	manualset3
196471	4	416049	7	NULL	NULL	0	NULL	precision	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Under optimum conditions , ascertained by evaluating various electrochemical parameters , the accuracy and precision ( 95 % ts ) were found to be + / - 0.3 % .
	manualset3
196472	5	416049	7	NULL	NULL	0	NULL	95 % ts	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Under optimum conditions , ascertained by evaluating various electrochemical parameters , the accuracy and precision ( 95 % ts ) were found to be + / - 0.3 % .
	manualset3
196473	6	416049	7	NULL	NULL	0	NULL	+ / - 0.3 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Under optimum conditions , ascertained by evaluating various electrochemical parameters , the accuracy and precision ( 95 % ts ) were found to be + / - 0.3 % .
	manualset3
196474	1	416050	7	NULL	NULL	0	NULL	 conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Under our conditions of acute heat exposure , hsp68 , 70 and their isoforms were globally distributed in all subcellular fractions examined , with a few notable exceptions in drug-treated cells .
	manualset3
196475	2	416050	7	NULL	NULL	0	NULL	acute heat exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Under our conditions of acute heat exposure , hsp68 , 70 and their isoforms were globally distributed in all subcellular fractions examined , with a few notable exceptions in drug-treated cells .
	manualset3
196476	3	416050	7	NULL	NULL	0	NULL	hsp68	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Under our conditions of acute heat exposure , hsp68 , 70 and their isoforms were globally distributed in all subcellular fractions examined , with a few notable exceptions in drug-treated cells .
	manualset3
196477	4	416050	7	NULL	NULL	0	NULL	hsp70	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Under our conditions of acute heat exposure , hsp68 , 70 and their isoforms were globally distributed in all subcellular fractions examined , with a few notable exceptions in drug-treated cells .
	manualset3
196478	5	416050	7	NULL	NULL	0	NULL	isoforms	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Under our conditions of acute heat exposure , hsp68 , 70 and their isoforms were globally distributed in all subcellular fractions examined , with a few notable exceptions in drug-treated cells .
	manualset3
196479	6	416050	7	NULL	NULL	0	NULL	subcellular fractions	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Under our conditions of acute heat exposure , hsp68 , 70 and their isoforms were globally distributed in all subcellular fractions examined , with a few notable exceptions in drug-treated cells .
	manualset3
196480	7	416050	7	NULL	NULL	0	NULL	notable exceptions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Under our conditions of acute heat exposure , hsp68 , 70 and their isoforms were globally distributed in all subcellular fractions examined , with a few notable exceptions in drug-treated cells .
	manualset3
196481	8	416050	7	NULL	NULL	0	NULL	drug-treated cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Under our conditions of acute heat exposure , hsp68 , 70 and their isoforms were globally distributed in all subcellular fractions examined , with a few notable exceptions in drug-treated cells .
	manualset3
196482	1	416051	7	NULL	NULL	0	NULL	scopy guided localization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Under scopy guided localization of the lumbar spine sympathetic blockade with local anesthetics to L2-5 vertebral levels were performed as a diagnostic block .
	manualset3
196483	2	416051	7	NULL	NULL	0	NULL	lumbar spine sympathetic blockade	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Under scopy guided localization of the lumbar spine sympathetic blockade with local anesthetics to L2-5 vertebral levels were performed as a diagnostic block .
	manualset3
196484	3	416051	7	NULL	NULL	0	NULL	local anesthetics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Under scopy guided localization of the lumbar spine sympathetic blockade with local anesthetics to L2-5 vertebral levels were performed as a diagnostic block .
	manualset3
196485	4	416051	7	NULL	NULL	0	NULL	L2-5 vertebral levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Under scopy guided localization of the lumbar spine sympathetic blockade with local anesthetics to L2-5 vertebral levels were performed as a diagnostic block .
	manualset3
196486	5	416051	7	NULL	NULL	0	NULL	diagnostic block 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Under scopy guided localization of the lumbar spine sympathetic blockade with local anesthetics to L2-5 vertebral levels were performed as a diagnostic block .
	manualset3
196487	1	416052	7	NULL	NULL	0	NULL	adjustment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After the adjustment was made for UR , more associations between the food groups and obesity status became apparent in both sexes .
	manualset3
196488	2	416052	7	NULL	NULL	0	NULL	UR	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	After the adjustment was made for UR , more associations between the food groups and obesity status became apparent in both sexes .
	manualset3
196489	3	416052	7	NULL	NULL	0	NULL	associations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	After the adjustment was made for UR , more associations between the food groups and obesity status became apparent in both sexes .
	manualset3
196490	4	416052	7	NULL	NULL	0	NULL	 food groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	After the adjustment was made for UR , more associations between the food groups and obesity status became apparent in both sexes .
	manualset3
196491	5	416052	7	NULL	NULL	0	NULL	obesity status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After the adjustment was made for UR , more associations between the food groups and obesity status became apparent in both sexes .
	manualset3
196492	6	416052	7	NULL	NULL	0	NULL	sexes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	After the adjustment was made for UR , more associations between the food groups and obesity status became apparent in both sexes .
	manualset3
196493	1	416053	7	NULL	NULL	0	NULL	 stoichiometric glucose limitation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Under stoichiometric glucose limitation , the glucose-to-cell yield increased and glucose-to-lactate yield decreased , indicating a metabolic shift .
	manualset3
196494	2	416053	7	NULL	NULL	0	NULL	glucose-to-cell yield	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Under stoichiometric glucose limitation , the glucose-to-cell yield increased and glucose-to-lactate yield decreased , indicating a metabolic shift .
	manualset3
196495	3	416053	7	NULL	NULL	0	NULL	glucose-to-lactate yield 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Under stoichiometric glucose limitation , the glucose-to-cell yield increased and glucose-to-lactate yield decreased , indicating a metabolic shift .
	manualset3
196496	4	416053	7	NULL	NULL	0	NULL	metabolic shift 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Under stoichiometric glucose limitation , the glucose-to-cell yield increased and glucose-to-lactate yield decreased , indicating a metabolic shift .
	manualset3
196497	1	416054	7	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Under such an hypothesis , the process of autonomy in adolescence involves a natural sequence of responses that seem to correspond to clinical syndromes .
	manualset3
196498	2	416054	7	NULL	NULL	0	NULL	process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Under such an hypothesis , the process of autonomy in adolescence involves a natural sequence of responses that seem to correspond to clinical syndromes .
	manualset3
196499	3	416054	7	NULL	NULL	0	NULL	autonomy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Under such an hypothesis , the process of autonomy in adolescence involves a natural sequence of responses that seem to correspond to clinical syndromes .
	manualset3
196500	4	416054	7	NULL	NULL	NULL	NULL	adolescence	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Under such an hypothesis , the process of autonomy in adolescence involves a natural sequence of responses that seem to correspond to clinical syndromes .
	manualset3
196501	5	416054	7	NULL	NULL	0	NULL	natural sequence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Under such an hypothesis , the process of autonomy in adolescence involves a natural sequence of responses that seem to correspond to clinical syndromes .
	manualset3
196502	6	416054	7	NULL	NULL	0	NULL	 responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Under such an hypothesis , the process of autonomy in adolescence involves a natural sequence of responses that seem to correspond to clinical syndromes .
	manualset3
196503	7	416054	7	NULL	NULL	0	NULL	clinical syndromes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Under such an hypothesis , the process of autonomy in adolescence involves a natural sequence of responses that seem to correspond to clinical syndromes .
	manualset3
196504	1	416055	7	NULL	NULL	0	NULL	 optimal condition	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Under the optimal condition , adsorption capacity of the P. putida 5-x cell to Cu2 + reached 87.3 mg x g ( -1 ) .
	manualset3
196505	2	416055	7	NULL	NULL	0	NULL	adsorption capacity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Under the optimal condition , adsorption capacity of the P. putida 5-x cell to Cu2 + reached 87.3 mg x g ( -1 ) .
	manualset3
196506	3	416055	7	NULL	NULL	0	NULL	P. putida 5-x cell 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Under the optimal condition , adsorption capacity of the P. putida 5-x cell to Cu2 + reached 87.3 mg x g ( -1 ) .
	manualset3
196507	4	416055	7	NULL	NULL	0	NULL	Cu2 +	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Under the optimal condition , adsorption capacity of the P. putida 5-x cell to Cu2 + reached 87.3 mg x g ( -1 ) .
	manualset3
196508	5	416055	7	NULL	NULL	0	NULL	87.3 mg x g ( -1 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Under the optimal condition , adsorption capacity of the P. putida 5-x cell to Cu2 + reached 87.3 mg x g ( -1 ) .
	manualset3
196509	1	416056	7	NULL	NULL	0	NULL	 conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Under the same conditions , however , the action of diphtheria toxin was completely inhibited by the amines .
	manualset3
196510	2	416056	7	NULL	NULL	0	NULL	action	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Under the same conditions , however , the action of diphtheria toxin was completely inhibited by the amines .
	manualset3
196511	3	416056	7	NULL	NULL	0	NULL	diphtheria toxin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Under the same conditions , however , the action of diphtheria toxin was completely inhibited by the amines .
	manualset3
196512	4	416056	7	NULL	NULL	0	NULL	 amines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Under the same conditions , however , the action of diphtheria toxin was completely inhibited by the amines .
	manualset3
196513	1	416057	7	NULL	NULL	0	NULL	experimental conditions 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Under the same experimental conditions any significant evidence of DNA repair was absent in primary hepatocytes from two human donors .
	manualset3
196514	2	416057	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Under the same experimental conditions any significant evidence of DNA repair was absent in primary hepatocytes from two human donors .
	manualset3
196515	3	416057	7	NULL	NULL	0	NULL	DNA repair	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Under the same experimental conditions any significant evidence of DNA repair was absent in primary hepatocytes from two human donors .
	manualset3
196516	4	416057	7	NULL	NULL	0	NULL	primary hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Under the same experimental conditions any significant evidence of DNA repair was absent in primary hepatocytes from two human donors .
	manualset3
196517	5	416057	7	NULL	NULL	0	NULL	 two human donors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Under the same experimental conditions any significant evidence of DNA repair was absent in primary hepatocytes from two human donors .
	manualset3
196518	1	416058	7	NULL	NULL	0	NULL	 tested conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Under the tested conditions , bacterial inactivation varied as a function of disinfectant type ( ranking by efficiency per mg of oxidant : ClO2 ) Cl2 ) ClNH2 ) and sample type ( bulk water vs. biofilm ) .
	manualset3
196519	2	416058	7	NULL	NULL	0	NULL	bacterial inactivation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Under the tested conditions , bacterial inactivation varied as a function of disinfectant type ( ranking by efficiency per mg of oxidant : ClO2 ) Cl2 ) ClNH2 ) and sample type ( bulk water vs. biofilm ) .
	manualset3
196520	3	416058	7	NULL	NULL	0	NULL	 function 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Under the tested conditions , bacterial inactivation varied as a function of disinfectant type ( ranking by efficiency per mg of oxidant : ClO2 ) Cl2 ) ClNH2 ) and sample type ( bulk water vs. biofilm ) .
	manualset3
196521	4	416058	7	NULL	NULL	0	NULL	 disinfectant type	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Under the tested conditions , bacterial inactivation varied as a function of disinfectant type ( ranking by efficiency per mg of oxidant : ClO2 ) Cl2 ) ClNH2 ) and sample type ( bulk water vs. biofilm ) .
	manualset3
196522	5	416058	7	NULL	NULL	0	NULL	ranking	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Under the tested conditions , bacterial inactivation varied as a function of disinfectant type ( ranking by efficiency per mg of oxidant : ClO2 ) Cl2 ) ClNH2 ) and sample type ( bulk water vs. biofilm ) .
	manualset3
196523	6	416058	7	NULL	NULL	0	NULL	efficiency per mg of oxidant	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Under the tested conditions , bacterial inactivation varied as a function of disinfectant type ( ranking by efficiency per mg of oxidant : ClO2 ) Cl2 ) ClNH2 ) and sample type ( bulk water vs. biofilm ) .
	manualset3
196524	7	416058	7	NULL	NULL	0	NULL	 ClO2 ) Cl2 ) ClNH2 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Under the tested conditions , bacterial inactivation varied as a function of disinfectant type ( ranking by efficiency per mg of oxidant : ClO2 ) Cl2 ) ClNH2 ) and sample type ( bulk water vs. biofilm ) .
	manualset3
196525	8	416058	7	NULL	NULL	0	NULL	sample type	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Under the tested conditions , bacterial inactivation varied as a function of disinfectant type ( ranking by efficiency per mg of oxidant : ClO2 ) Cl2 ) ClNH2 ) and sample type ( bulk water vs. biofilm ) .
	manualset3
196526	9	416058	7	NULL	NULL	0	NULL	bulk water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Under the tested conditions , bacterial inactivation varied as a function of disinfectant type ( ranking by efficiency per mg of oxidant : ClO2 ) Cl2 ) ClNH2 ) and sample type ( bulk water vs. biofilm ) .
	manualset3
196527	10	416058	7	NULL	NULL	0	NULL	biofilm 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Under the tested conditions , bacterial inactivation varied as a function of disinfectant type ( ranking by efficiency per mg of oxidant : ClO2 ) Cl2 ) ClNH2 ) and sample type ( bulk water vs. biofilm ) .
	manualset3
196528	1	416059	7	NULL	NULL	0	NULL	conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Under these conditions , Rp-adenosine-3 ' , 5 ' - cyclic monophosphorothioate triethylammonium , but not ZD7288 , altered the FSK-induced response of GnRH-1 neurons .
	manualset3
196529	2	416059	7	NULL	NULL	0	NULL	Rp-adenosine-3 ' , 5 ' - cyclic monophosphorothioate triethylammonium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Under these conditions , Rp-adenosine-3 ' , 5 ' - cyclic monophosphorothioate triethylammonium , but not ZD7288 , altered the FSK-induced response of GnRH-1 neurons .
	manualset3
196530	3	416059	7	NULL	NULL	0	NULL	ZD7288	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Under these conditions , Rp-adenosine-3 ' , 5 ' - cyclic monophosphorothioate triethylammonium , but not ZD7288 , altered the FSK-induced response of GnRH-1 neurons .
	manualset3
196531	4	416059	7	NULL	NULL	0	NULL	FSK-induced response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Under these conditions , Rp-adenosine-3 ' , 5 ' - cyclic monophosphorothioate triethylammonium , but not ZD7288 , altered the FSK-induced response of GnRH-1 neurons .
	manualset3
196532	5	416059	7	NULL	NULL	0	NULL	GnRH-1 neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Under these conditions , Rp-adenosine-3 ' , 5 ' - cyclic monophosphorothioate triethylammonium , but not ZD7288 , altered the FSK-induced response of GnRH-1 neurons .
	manualset3
196533	1	416060	7	NULL	NULL	0	NULL	cholangitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	After the cholangitis subsided , ESWL was performed under the direct cholangiography through ENBD and PTBD and excellent results were obtained which are herein reported .
	manualset3
196534	2	416060	7	NULL	NULL	0	NULL	ESWL	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After the cholangitis subsided , ESWL was performed under the direct cholangiography through ENBD and PTBD and excellent results were obtained which are herein reported .
	manualset3
196535	3	416060	7	NULL	NULL	0	NULL	 direct cholangiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After the cholangitis subsided , ESWL was performed under the direct cholangiography through ENBD and PTBD and excellent results were obtained which are herein reported .
	manualset3
196536	4	416060	7	NULL	NULL	0	NULL	ENBD	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After the cholangitis subsided , ESWL was performed under the direct cholangiography through ENBD and PTBD and excellent results were obtained which are herein reported .
	manualset3
196537	5	416060	7	NULL	NULL	0	NULL	PTBD	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After the cholangitis subsided , ESWL was performed under the direct cholangiography through ENBD and PTBD and excellent results were obtained which are herein reported .
	manualset3
196538	6	416060	7	NULL	NULL	0	NULL	excellent results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After the cholangitis subsided , ESWL was performed under the direct cholangiography through ENBD and PTBD and excellent results were obtained which are herein reported .
	manualset3
196539	1	416061	7	NULL	NULL	0	NULL	conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Under these conditions , we found that mRNA and protein for CHOP/GADD153 , a C/EBP family transcription factor that is involved in ER stress-induced apoptosis , were induced .
	manualset3
196540	2	416061	7	NULL	NULL	0	NULL	mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Under these conditions , we found that mRNA and protein for CHOP/GADD153 , a C/EBP family transcription factor that is involved in ER stress-induced apoptosis , were induced .
	manualset3
196541	3	416061	7	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Under these conditions , we found that mRNA and protein for CHOP/GADD153 , a C/EBP family transcription factor that is involved in ER stress-induced apoptosis , were induced .
	manualset3
196542	4	416061	7	NULL	NULL	0	NULL	CHOP/GADD153	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Under these conditions , we found that mRNA and protein for CHOP/GADD153 , a C/EBP family transcription factor that is involved in ER stress-induced apoptosis , were induced .
	manualset3
196543	5	416061	7	NULL	NULL	0	NULL	C/EBP family transcription factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Under these conditions , we found that mRNA and protein for CHOP/GADD153 , a C/EBP family transcription factor that is involved in ER stress-induced apoptosis , were induced .
	manualset3
196544	6	416061	7	NULL	NULL	0	NULL	ER stress-induced apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Under these conditions , we found that mRNA and protein for CHOP/GADD153 , a C/EBP family transcription factor that is involved in ER stress-induced apoptosis , were induced .
	manualset3
196545	1	416062	7	NULL	NULL	0	NULL	exposure conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Under these exposure conditions , neither microwave nor RF radiation had a detectable effect on stress protein induction as determined by either comparison of RF-exposed cells with sham-exposed cells or comparison with heat-stressed or Cd + + positive control cells .
	manualset3
196546	2	416062	7	NULL	NULL	0	NULL	microwave radiation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Under these exposure conditions , neither microwave nor RF radiation had a detectable effect on stress protein induction as determined by either comparison of RF-exposed cells with sham-exposed cells or comparison with heat-stressed or Cd + + positive control cells .
	manualset3
196547	3	416062	7	NULL	NULL	0	NULL	RF radiation 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Under these exposure conditions , neither microwave nor RF radiation had a detectable effect on stress protein induction as determined by either comparison of RF-exposed cells with sham-exposed cells or comparison with heat-stressed or Cd + + positive control cells .
	manualset3
196548	4	416062	7	NULL	NULL	0	NULL	detectable effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Under these exposure conditions , neither microwave nor RF radiation had a detectable effect on stress protein induction as determined by either comparison of RF-exposed cells with sham-exposed cells or comparison with heat-stressed or Cd + + positive control cells .
	manualset3
196549	5	416062	7	NULL	NULL	0	NULL	stress protein induction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Under these exposure conditions , neither microwave nor RF radiation had a detectable effect on stress protein induction as determined by either comparison of RF-exposed cells with sham-exposed cells or comparison with heat-stressed or Cd + + positive control cells .
	manualset3
196550	6	416062	7	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Under these exposure conditions , neither microwave nor RF radiation had a detectable effect on stress protein induction as determined by either comparison of RF-exposed cells with sham-exposed cells or comparison with heat-stressed or Cd + + positive control cells .
	manualset3
196551	7	416062	7	NULL	NULL	0	NULL	RF-exposed cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Under these exposure conditions , neither microwave nor RF radiation had a detectable effect on stress protein induction as determined by either comparison of RF-exposed cells with sham-exposed cells or comparison with heat-stressed or Cd + + positive control cells .
	manualset3
196552	8	416062	7	NULL	NULL	0	NULL	sham-exposed cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Under these exposure conditions , neither microwave nor RF radiation had a detectable effect on stress protein induction as determined by either comparison of RF-exposed cells with sham-exposed cells or comparison with heat-stressed or Cd + + positive control cells .
	manualset3
196553	9	416062	7	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Under these exposure conditions , neither microwave nor RF radiation had a detectable effect on stress protein induction as determined by either comparison of RF-exposed cells with sham-exposed cells or comparison with heat-stressed or Cd + + positive control cells .
	manualset3
196554	10	416062	7	NULL	NULL	0	NULL	 heat-stressed control cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Under these exposure conditions , neither microwave nor RF radiation had a detectable effect on stress protein induction as determined by either comparison of RF-exposed cells with sham-exposed cells or comparison with heat-stressed or Cd + + positive control cells .
	manualset3
196555	11	416062	7	NULL	NULL	0	NULL	 Cd + + positive control cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Under these exposure conditions , neither microwave nor RF radiation had a detectable effect on stress protein induction as determined by either comparison of RF-exposed cells with sham-exposed cells or comparison with heat-stressed or Cd + + positive control cells .
	manualset3
196556	1	416063	7	NULL	NULL	0	NULL	condition	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Under this condition , a maximum concentration of 300 mg/l of rhG-CSF and the expression yield of 0.6 mg of rhG-CSF/g of methanol were attained .
	manualset3
196557	2	416063	7	NULL	NULL	0	NULL	maximum concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Under this condition , a maximum concentration of 300 mg/l of rhG-CSF and the expression yield of 0.6 mg of rhG-CSF/g of methanol were attained .
	manualset3
196558	3	416063	7	NULL	NULL	NULL	NULL	300 mg/l 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Under this condition , a maximum concentration of 300 mg/l of rhG-CSF and the expression yield of 0.6 mg of rhG-CSF/g of methanol were attained .
	manualset3
196559	4	416063	7	NULL	NULL	NULL	NULL	rhG-CSF 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Under this condition , a maximum concentration of 300 mg/l of rhG-CSF and the expression yield of 0.6 mg of rhG-CSF/g of methanol were attained .
	manualset3
196560	5	416063	7	NULL	NULL	NULL	NULL	expression yield	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Under this condition , a maximum concentration of 300 mg/l of rhG-CSF and the expression yield of 0.6 mg of rhG-CSF/g of methanol were attained .
	manualset3
196561	6	416063	7	NULL	NULL	NULL	NULL	 0.6 mg 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Under this condition , a maximum concentration of 300 mg/l of rhG-CSF and the expression yield of 0.6 mg of rhG-CSF/g of methanol were attained .
	manualset3
196562	7	416063	7	NULL	NULL	NULL	NULL	 rhG-CSF/g of methanol 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Under this condition , a maximum concentration of 300 mg/l of rhG-CSF and the expression yield of 0.6 mg of rhG-CSF/g of methanol were attained .
	manualset3
196564	1	416064	7	NULL	NULL	0	NULL	condition	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Under this condition , the analysis of DNA may be useless .
	manualset3
196565	2	416064	7	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Under this condition , the analysis of DNA may be useless .
	manualset3
196566	3	416064	7	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Under this condition , the analysis of DNA may be useless .
	manualset3
196567	1	416065	7	NULL	NULL	0	NULL	Understanding breastfeeding initiation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Understanding breastfeeding initiation and continuation in rural communities : a combined qualitative/quantitative approach .
	manualset3
196568	2	416065	7	NULL	NULL	0	NULL	continuation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Understanding breastfeeding initiation and continuation in rural communities : a combined qualitative/quantitative approach .
	manualset3
196569	3	416065	7	NULL	NULL	0	NULL	rural communities	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Understanding breastfeeding initiation and continuation in rural communities : a combined qualitative/quantitative approach .
	manualset3
196570	4	416065	7	NULL	NULL	0	NULL	combined qualitative/quantitative approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Understanding breastfeeding initiation and continuation in rural communities : a combined qualitative/quantitative approach .
	manualset3
196571	1	416066	7	NULL	NULL	0	NULL	Understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Understanding how neural mechanisms implicated in impulse control are affected by addictive drugs may therefore prove a useful strategy in the search for new treatment options .
	manualset3
196572	2	416066	7	NULL	NULL	0	NULL	neural mechanisms	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Understanding how neural mechanisms implicated in impulse control are affected by addictive drugs may therefore prove a useful strategy in the search for new treatment options .
	manualset3
196573	3	416066	7	NULL	NULL	0	NULL	 impulse control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Understanding how neural mechanisms implicated in impulse control are affected by addictive drugs may therefore prove a useful strategy in the search for new treatment options .
	manualset3
196574	4	416066	7	NULL	NULL	0	NULL	addictive drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Understanding how neural mechanisms implicated in impulse control are affected by addictive drugs may therefore prove a useful strategy in the search for new treatment options .
	manualset3
196575	5	416066	7	NULL	NULL	0	NULL	 strategy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Understanding how neural mechanisms implicated in impulse control are affected by addictive drugs may therefore prove a useful strategy in the search for new treatment options .
	manualset3
196576	6	416066	7	NULL	NULL	0	NULL	search	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Understanding how neural mechanisms implicated in impulse control are affected by addictive drugs may therefore prove a useful strategy in the search for new treatment options .
	manualset3
196577	7	416066	7	NULL	NULL	0	NULL	new treatment options	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Understanding how neural mechanisms implicated in impulse control are affected by addictive drugs may therefore prove a useful strategy in the search for new treatment options .
	manualset3
196578	1	416067	7	NULL	NULL	0	NULL	5-year follow-up study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( 5-year follow-up study on 600 cases treated by the Schauta-Amreich operation ) .
	manualset3
196579	2	416067	7	NULL	NULL	0	NULL	600 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( 5-year follow-up study on 600 cases treated by the Schauta-Amreich operation ) .
	manualset3
196580	3	416067	7	NULL	NULL	0	NULL	Schauta-Amreich operation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( 5-year follow-up study on 600 cases treated by the Schauta-Amreich operation ) .
	manualset3
196581	1	416068	7	NULL	NULL	0	NULL	Congenital cystic dilation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Congenital cystic dilation of the choledochus ) .
	manualset3
196582	2	416068	7	NULL	NULL	0	NULL	choledochus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Congenital cystic dilation of the choledochus ) .
	manualset3
196583	1	416069	7	NULL	NULL	0	NULL	Understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Understanding silibinin 's modes of action against HCV using viral kinetic modeling .
	manualset3
196584	2	416069	7	NULL	NULL	0	NULL	silibinin 's modes of action	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Understanding silibinin 's modes of action against HCV using viral kinetic modeling .
	manualset3
196585	3	416069	7	NULL	NULL	0	NULL	HCV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Understanding silibinin 's modes of action against HCV using viral kinetic modeling .
	manualset3
196586	4	416069	7	NULL	NULL	0	NULL	viral kinetic modeling	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Understanding silibinin 's modes of action against HCV using viral kinetic modeling .
	manualset3
196587	1	416070	7	NULL	NULL	0	NULL	radiographs	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Undertaking radiographs significantly lengthened delays from presentation to referral .
	manualset3
196588	2	416070	7	NULL	NULL	0	NULL	lengthened delays 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Undertaking radiographs significantly lengthened delays from presentation to referral .
	manualset3
196589	3	416070	7	NULL	NULL	0	NULL	presentation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Undertaking radiographs significantly lengthened delays from presentation to referral .
	manualset3
196590	4	416070	7	NULL	NULL	0	NULL	referral	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Undertaking radiographs significantly lengthened delays from presentation to referral .
	manualset3
196591	1	416071	7	NULL	NULL	0	NULL	Unexpected temperature dependence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Unexpected temperature dependence of potassium release from the isolated perfused rat liver .
	manualset3
196592	2	416071	7	NULL	NULL	0	NULL	potassium release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unexpected temperature dependence of potassium release from the isolated perfused rat liver .
	manualset3
196593	3	416071	7	NULL	NULL	0	NULL	 isolated perfused rat liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Unexpected temperature dependence of potassium release from the isolated perfused rat liver .
	manualset3
196594	1	416072	7	NULL	NULL	0	NULL	Unexpected tumor progression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unexpected tumor progression after conization for carcinoma in situ of the uterine cervix .
	manualset3
196595	2	416072	7	NULL	NULL	0	NULL	conization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unexpected tumor progression after conization for carcinoma in situ of the uterine cervix .
	manualset3
196596	3	416072	7	NULL	NULL	0	NULL	carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Unexpected tumor progression after conization for carcinoma in situ of the uterine cervix .
	manualset3
196597	4	416072	7	NULL	NULL	0	NULL	uterine cervix	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Unexpected tumor progression after conization for carcinoma in situ of the uterine cervix .
	manualset3
196598	1	416073	7	NULL	NULL	0	NULL	Unfertilized oocyte supernatant 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfertilized oocyte supernatant exhibited phosphatidylinositol and phosphatidylethanolamine transfer activity also , but at the late blastula stage the former had dropped 18-fold and the latter was no longer detectable under our assay conditions .
	manualset3
196599	2	416073	7	NULL	NULL	0	NULL	 phosphatidylinositol transfer activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfertilized oocyte supernatant exhibited phosphatidylinositol and phosphatidylethanolamine transfer activity also , but at the late blastula stage the former had dropped 18-fold and the latter was no longer detectable under our assay conditions .
	manualset3
196600	3	416073	7	NULL	NULL	0	NULL	phosphatidylethanolamine transfer activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfertilized oocyte supernatant exhibited phosphatidylinositol and phosphatidylethanolamine transfer activity also , but at the late blastula stage the former had dropped 18-fold and the latter was no longer detectable under our assay conditions .
	manualset3
196601	4	416073	7	NULL	NULL	0	NULL	late blastula stage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfertilized oocyte supernatant exhibited phosphatidylinositol and phosphatidylethanolamine transfer activity also , but at the late blastula stage the former had dropped 18-fold and the latter was no longer detectable under our assay conditions .
	manualset3
196602	5	416073	7	NULL	NULL	0	NULL	18-fold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfertilized oocyte supernatant exhibited phosphatidylinositol and phosphatidylethanolamine transfer activity also , but at the late blastula stage the former had dropped 18-fold and the latter was no longer detectable under our assay conditions .
	manualset3
196603	6	416073	7	NULL	NULL	0	NULL	assay conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfertilized oocyte supernatant exhibited phosphatidylinositol and phosphatidylethanolamine transfer activity also , but at the late blastula stage the former had dropped 18-fold and the latter was no longer detectable under our assay conditions .
	manualset3
196604	1	416074	7	NULL	NULL	0	NULL	development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After the development of mechanical hyperalgesia in the neuropathic limb , the responses of medial bulboreticular neurons to noxious skin stimulation were determined , and the attenuation of the responses was attempted by administering systemically medetomidine , a highly specific alpha 2-adrenoceptor agonist .
	manualset3
196605	2	416074	7	NULL	NULL	0	NULL	mechanical hyperalgesia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After the development of mechanical hyperalgesia in the neuropathic limb , the responses of medial bulboreticular neurons to noxious skin stimulation were determined , and the attenuation of the responses was attempted by administering systemically medetomidine , a highly specific alpha 2-adrenoceptor agonist .
	manualset3
196606	3	416074	7	NULL	NULL	0	NULL	neuropathic limb	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After the development of mechanical hyperalgesia in the neuropathic limb , the responses of medial bulboreticular neurons to noxious skin stimulation were determined , and the attenuation of the responses was attempted by administering systemically medetomidine , a highly specific alpha 2-adrenoceptor agonist .
	manualset3
196607	4	416074	7	NULL	NULL	0	NULL	responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After the development of mechanical hyperalgesia in the neuropathic limb , the responses of medial bulboreticular neurons to noxious skin stimulation were determined , and the attenuation of the responses was attempted by administering systemically medetomidine , a highly specific alpha 2-adrenoceptor agonist .
	manualset3
196608	5	416074	7	NULL	NULL	0	NULL	medial bulboreticular neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	After the development of mechanical hyperalgesia in the neuropathic limb , the responses of medial bulboreticular neurons to noxious skin stimulation were determined , and the attenuation of the responses was attempted by administering systemically medetomidine , a highly specific alpha 2-adrenoceptor agonist .
	manualset3
196609	6	416074	7	NULL	NULL	0	NULL	noxious skin stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After the development of mechanical hyperalgesia in the neuropathic limb , the responses of medial bulboreticular neurons to noxious skin stimulation were determined , and the attenuation of the responses was attempted by administering systemically medetomidine , a highly specific alpha 2-adrenoceptor agonist .
	manualset3
196610	7	416074	7	NULL	NULL	0	NULL	attenuation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After the development of mechanical hyperalgesia in the neuropathic limb , the responses of medial bulboreticular neurons to noxious skin stimulation were determined , and the attenuation of the responses was attempted by administering systemically medetomidine , a highly specific alpha 2-adrenoceptor agonist .
	manualset3
196611	8	416074	7	NULL	NULL	0	NULL	responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After the development of mechanical hyperalgesia in the neuropathic limb , the responses of medial bulboreticular neurons to noxious skin stimulation were determined , and the attenuation of the responses was attempted by administering systemically medetomidine , a highly specific alpha 2-adrenoceptor agonist .
	manualset3
196612	9	416074	7	NULL	NULL	0	NULL	medetomidine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	After the development of mechanical hyperalgesia in the neuropathic limb , the responses of medial bulboreticular neurons to noxious skin stimulation were determined , and the attenuation of the responses was attempted by administering systemically medetomidine , a highly specific alpha 2-adrenoceptor agonist .
	manualset3
196613	10	416074	7	NULL	NULL	0	NULL	alpha 2-adrenoceptor agonist	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After the development of mechanical hyperalgesia in the neuropathic limb , the responses of medial bulboreticular neurons to noxious skin stimulation were determined , and the attenuation of the responses was attempted by administering systemically medetomidine , a highly specific alpha 2-adrenoceptor agonist .
	manualset3
196614	1	416075	7	NULL	NULL	0	NULL	Unfolding	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfolding of the III-1 module on the cell surface may control matrix assembly site expression and represent an important step in the initiation of cell-dependent fibronectin polymerization .
	manualset3
196615	2	416075	7	NULL	NULL	0	NULL	 III-1 module	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfolding of the III-1 module on the cell surface may control matrix assembly site expression and represent an important step in the initiation of cell-dependent fibronectin polymerization .
	manualset3
196616	3	416075	7	NULL	NULL	0	NULL	cell surface	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfolding of the III-1 module on the cell surface may control matrix assembly site expression and represent an important step in the initiation of cell-dependent fibronectin polymerization .
	manualset3
196617	4	416075	7	NULL	NULL	0	NULL	matrix assembly site expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfolding of the III-1 module on the cell surface may control matrix assembly site expression and represent an important step in the initiation of cell-dependent fibronectin polymerization .
	manualset3
196618	5	416075	7	NULL	NULL	0	NULL	important step	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfolding of the III-1 module on the cell surface may control matrix assembly site expression and represent an important step in the initiation of cell-dependent fibronectin polymerization .
	manualset3
196619	6	416075	7	NULL	NULL	0	NULL	 initiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfolding of the III-1 module on the cell surface may control matrix assembly site expression and represent an important step in the initiation of cell-dependent fibronectin polymerization .
	manualset3
196620	7	416075	7	NULL	NULL	0	NULL	cell-dependent fibronectin polymerization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfolding of the III-1 module on the cell surface may control matrix assembly site expression and represent an important step in the initiation of cell-dependent fibronectin polymerization .
	manualset3
196621	1	416076	7	NULL	NULL	0	NULL	competing hydrolysis reaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfortunately , a competing hydrolysis reaction reduces the lifetime of the intermediate precluding its trapping and identification .
	manualset3
196622	2	416076	7	NULL	NULL	0	NULL	lifetime	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfortunately , a competing hydrolysis reaction reduces the lifetime of the intermediate precluding its trapping and identification .
	manualset3
196623	3	416076	7	NULL	NULL	0	NULL	intermediate	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfortunately , a competing hydrolysis reaction reduces the lifetime of the intermediate precluding its trapping and identification .
	manualset3
196624	4	416076	7	NULL	NULL	0	NULL	trapping	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfortunately , a competing hydrolysis reaction reduces the lifetime of the intermediate precluding its trapping and identification .
	manualset3
196625	5	416076	7	NULL	NULL	0	NULL	identification	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfortunately , a competing hydrolysis reaction reduces the lifetime of the intermediate precluding its trapping and identification .
	manualset3
196626	1	416077	7	NULL	NULL	0	NULL	diagnostic tests	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfortunately , there are no reliable diagnostic tests distinguishing fungal infection and colonization .
	manualset3
196627	2	416077	7	NULL	NULL	0	NULL	 fungal infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfortunately , there are no reliable diagnostic tests distinguishing fungal infection and colonization .
	manualset3
196628	3	416077	7	NULL	NULL	0	NULL	colonization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfortunately , there are no reliable diagnostic tests distinguishing fungal infection and colonization .
	manualset3
196629	1	416078	7	NULL	NULL	0	NULL	Unilateal injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Unilateal injection of the drug induced degenerative changes in the injected testis only ; the contralateral testis appeared normal macroscopically and histologically .
	manualset3
196630	2	416078	7	NULL	NULL	0	NULL	drug 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Unilateal injection of the drug induced degenerative changes in the injected testis only ; the contralateral testis appeared normal macroscopically and histologically .
	manualset3
196631	3	416078	7	NULL	NULL	0	NULL	degenerative changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unilateal injection of the drug induced degenerative changes in the injected testis only ; the contralateral testis appeared normal macroscopically and histologically .
	manualset3
196632	4	416078	7	NULL	NULL	0	NULL	injected testis 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Unilateal injection of the drug induced degenerative changes in the injected testis only ; the contralateral testis appeared normal macroscopically and histologically .
	manualset3
196633	5	416078	7	NULL	NULL	0	NULL	contralateral testis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Unilateal injection of the drug induced degenerative changes in the injected testis only ; the contralateral testis appeared normal macroscopically and histologically .
	manualset3
196634	1	416079	7	NULL	NULL	NULL	NULL	failure	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After the failure of ENHANCEd cholesterol lowering in familial hypercholesterolemia , SEAS of problems with ezetimibe .
	manualset3
196635	2	416079	7	NULL	NULL	0	NULL	ENHANCEd cholesterol lowering	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After the failure of ENHANCEd cholesterol lowering in familial hypercholesterolemia , SEAS of problems with ezetimibe .
	manualset3
196636	3	416079	7	NULL	NULL	0	NULL	familial hypercholesterolemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	After the failure of ENHANCEd cholesterol lowering in familial hypercholesterolemia , SEAS of problems with ezetimibe .
	manualset3
196637	4	416079	7	NULL	NULL	NULL	NULL	SEAS of problems	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After the failure of ENHANCEd cholesterol lowering in familial hypercholesterolemia , SEAS of problems with ezetimibe .
	manualset3
196639	6	416079	7	NULL	NULL	0	NULL	ezetimibe	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	After the failure of ENHANCEd cholesterol lowering in familial hypercholesterolemia , SEAS of problems with ezetimibe .
	manualset3
196640	1	416080	7	NULL	NULL	0	NULL	Unilateral nephrectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Unilateral nephrectomy , when performed during this period of natural increase , induced the formation of supplementary nephrons in the contralateral kidney .
	manualset3
196641	2	416080	7	NULL	NULL	0	NULL	period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Unilateral nephrectomy , when performed during this period of natural increase , induced the formation of supplementary nephrons in the contralateral kidney .
	manualset3
196642	3	416080	7	NULL	NULL	0	NULL	 formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unilateral nephrectomy , when performed during this period of natural increase , induced the formation of supplementary nephrons in the contralateral kidney .
	manualset3
196643	4	416080	7	NULL	NULL	0	NULL	supplementary nephrons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Unilateral nephrectomy , when performed during this period of natural increase , induced the formation of supplementary nephrons in the contralateral kidney .
	manualset3
196644	5	416080	7	NULL	NULL	0	NULL	contralateral kidney	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Unilateral nephrectomy , when performed during this period of natural increase , induced the formation of supplementary nephrons in the contralateral kidney .
	manualset3
198170	6	416080	7	NULL	NULL	0	NULL	natural increase	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Unilateral nephrectomy , when performed during this period of natural increase , induced the formation of supplementary nephrons in the contralateral kidney .
	manualset3
196645	1	416081	7	NULL	NULL	0	NULL	Unilateral paroxysmal diaphragmatic flutter	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Unilateral paroxysmal diaphragmatic flutter : response to quinidine .
	manualset3
196646	2	416081	7	NULL	NULL	0	NULL	 response 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Unilateral paroxysmal diaphragmatic flutter : response to quinidine .
	manualset3
196647	3	416081	7	NULL	NULL	0	NULL	quinidine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Unilateral paroxysmal diaphragmatic flutter : response to quinidine .
	manualset3
196648	1	416082	7	NULL	NULL	0	NULL	Unilateral tecto-pretectal lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Unilateral tecto-pretectal lesions performed at birth lead to extensive retrograde degeneration of contralaterally projecting ganglion cells in the opposite retina : but both the ipsilateral terminal fields of the same retina and its population of ipsilaterally projecting ganglion cells are increased .
	manualset3
196649	2	416082	7	NULL	NULL	0	NULL	 birth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unilateral tecto-pretectal lesions performed at birth lead to extensive retrograde degeneration of contralaterally projecting ganglion cells in the opposite retina : but both the ipsilateral terminal fields of the same retina and its population of ipsilaterally projecting ganglion cells are increased .
	manualset3
196650	3	416082	7	NULL	NULL	0	NULL	extensive retrograde degeneration 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unilateral tecto-pretectal lesions performed at birth lead to extensive retrograde degeneration of contralaterally projecting ganglion cells in the opposite retina : but both the ipsilateral terminal fields of the same retina and its population of ipsilaterally projecting ganglion cells are increased .
	manualset3
196651	4	416082	7	NULL	NULL	0	NULL	contralaterally projecting ganglion cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Unilateral tecto-pretectal lesions performed at birth lead to extensive retrograde degeneration of contralaterally projecting ganglion cells in the opposite retina : but both the ipsilateral terminal fields of the same retina and its population of ipsilaterally projecting ganglion cells are increased .
	manualset3
196652	5	416082	7	NULL	NULL	0	NULL	opposite retina 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Unilateral tecto-pretectal lesions performed at birth lead to extensive retrograde degeneration of contralaterally projecting ganglion cells in the opposite retina : but both the ipsilateral terminal fields of the same retina and its population of ipsilaterally projecting ganglion cells are increased .
	manualset3
196653	6	416082	7	NULL	NULL	0	NULL	ipsilateral terminal fields	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Unilateral tecto-pretectal lesions performed at birth lead to extensive retrograde degeneration of contralaterally projecting ganglion cells in the opposite retina : but both the ipsilateral terminal fields of the same retina and its population of ipsilaterally projecting ganglion cells are increased .
	manualset3
196654	7	416082	7	NULL	NULL	0	NULL	same retina 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Unilateral tecto-pretectal lesions performed at birth lead to extensive retrograde degeneration of contralaterally projecting ganglion cells in the opposite retina : but both the ipsilateral terminal fields of the same retina and its population of ipsilaterally projecting ganglion cells are increased .
	manualset3
196655	8	416082	7	NULL	NULL	0	NULL	population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Unilateral tecto-pretectal lesions performed at birth lead to extensive retrograde degeneration of contralaterally projecting ganglion cells in the opposite retina : but both the ipsilateral terminal fields of the same retina and its population of ipsilaterally projecting ganglion cells are increased .
	manualset3
196656	9	416082	7	NULL	NULL	0	NULL	ipsilaterally projecting ganglion cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Unilateral tecto-pretectal lesions performed at birth lead to extensive retrograde degeneration of contralaterally projecting ganglion cells in the opposite retina : but both the ipsilateral terminal fields of the same retina and its population of ipsilaterally projecting ganglion cells are increased .
	manualset3
196657	1	416083	7	NULL	NULL	0	NULL	Uninfected cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Uninfected cells expressing A56 and K2 exhibited resistance to fusing with A56 mutant virus-infected cells , whereas expression of A56 or K2 alone induced little or no resistance , which fits with the need for both proteins to bind the EFC .
	manualset3
196658	2	416083	7	NULL	NULL	0	NULL	A56	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Uninfected cells expressing A56 and K2 exhibited resistance to fusing with A56 mutant virus-infected cells , whereas expression of A56 or K2 alone induced little or no resistance , which fits with the need for both proteins to bind the EFC .
	manualset3
196659	3	416083	7	NULL	NULL	0	NULL	K2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Uninfected cells expressing A56 and K2 exhibited resistance to fusing with A56 mutant virus-infected cells , whereas expression of A56 or K2 alone induced little or no resistance , which fits with the need for both proteins to bind the EFC .
	manualset3
196660	4	416083	7	NULL	NULL	0	NULL	A56 mutant virus-infected cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Uninfected cells expressing A56 and K2 exhibited resistance to fusing with A56 mutant virus-infected cells , whereas expression of A56 or K2 alone induced little or no resistance , which fits with the need for both proteins to bind the EFC .
	manualset3
196661	5	416083	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Uninfected cells expressing A56 and K2 exhibited resistance to fusing with A56 mutant virus-infected cells , whereas expression of A56 or K2 alone induced little or no resistance , which fits with the need for both proteins to bind the EFC .
	manualset3
196662	6	416083	7	NULL	NULL	0	NULL	A56	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Uninfected cells expressing A56 and K2 exhibited resistance to fusing with A56 mutant virus-infected cells , whereas expression of A56 or K2 alone induced little or no resistance , which fits with the need for both proteins to bind the EFC .
	manualset3
196663	7	416083	7	NULL	NULL	0	NULL	K2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Uninfected cells expressing A56 and K2 exhibited resistance to fusing with A56 mutant virus-infected cells , whereas expression of A56 or K2 alone induced little or no resistance , which fits with the need for both proteins to bind the EFC .
	manualset3
196664	8	416083	7	NULL	NULL	0	NULL	proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Uninfected cells expressing A56 and K2 exhibited resistance to fusing with A56 mutant virus-infected cells , whereas expression of A56 or K2 alone induced little or no resistance , which fits with the need for both proteins to bind the EFC .
	manualset3
196665	9	416083	7	NULL	NULL	0	NULL	 EFC	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Uninfected cells expressing A56 and K2 exhibited resistance to fusing with A56 mutant virus-infected cells , whereas expression of A56 or K2 alone induced little or no resistance , which fits with the need for both proteins to bind the EFC .
	manualset3
196666	1	416084	7	NULL	NULL	0	NULL	biochemical activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unique biochemical , cytotoxic , and antitumor activity of camptothecin and 4beta-amino-4 ' - O-demethylepipodophyllotoxin conjugates .
	manualset3
196667	2	416084	7	NULL	NULL	0	NULL	cytotoxic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unique biochemical , cytotoxic , and antitumor activity of camptothecin and 4beta-amino-4 ' - O-demethylepipodophyllotoxin conjugates .
	manualset3
196668	3	416084	7	NULL	NULL	0	NULL	antitumor activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unique biochemical , cytotoxic , and antitumor activity of camptothecin and 4beta-amino-4 ' - O-demethylepipodophyllotoxin conjugates .
	manualset3
196669	4	416084	7	NULL	NULL	0	NULL	camptothecin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Unique biochemical , cytotoxic , and antitumor activity of camptothecin and 4beta-amino-4 ' - O-demethylepipodophyllotoxin conjugates .
	manualset3
196670	5	416084	7	NULL	NULL	0	NULL	4beta-amino-4 ' - O-demethylepipodophyllotoxin conjugates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Unique biochemical , cytotoxic , and antitumor activity of camptothecin and 4beta-amino-4 ' - O-demethylepipodophyllotoxin conjugates .
	manualset3
196671	1	416085	7	NULL	NULL	0	NULL	Unique spectra	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Unique spectra are defined for various sites in the mouth and are likely related to the degree of keratinization .
	manualset3
196672	2	416085	7	NULL	NULL	0	NULL	various sites	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Unique spectra are defined for various sites in the mouth and are likely related to the degree of keratinization .
	manualset3
196673	3	416085	7	NULL	NULL	0	NULL	mouth	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Unique spectra are defined for various sites in the mouth and are likely related to the degree of keratinization .
	manualset3
196674	4	416085	7	NULL	NULL	0	NULL	 degree	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Unique spectra are defined for various sites in the mouth and are likely related to the degree of keratinization .
	manualset3
196675	5	416085	7	NULL	NULL	0	NULL	keratinization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unique spectra are defined for various sites in the mouth and are likely related to the degree of keratinization .
	manualset3
196676	1	416086	7	NULL	NULL	0	NULL	first course	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After the first course of high-dose Ara-C containing consolidation therapy , the patient developed multiple skin lesions on the left foot .
	manualset3
196677	2	416086	7	NULL	NULL	0	NULL	high-dose Ara-C	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After the first course of high-dose Ara-C containing consolidation therapy , the patient developed multiple skin lesions on the left foot .
	manualset3
196678	3	416086	7	NULL	NULL	0	NULL	consolidation therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After the first course of high-dose Ara-C containing consolidation therapy , the patient developed multiple skin lesions on the left foot .
	manualset3
196679	4	416086	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	After the first course of high-dose Ara-C containing consolidation therapy , the patient developed multiple skin lesions on the left foot .
	manualset3
196680	5	416086	7	NULL	NULL	0	NULL	multiple skin lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After the first course of high-dose Ara-C containing consolidation therapy , the patient developed multiple skin lesions on the left foot .
	manualset3
196681	6	416086	7	NULL	NULL	0	NULL	left foot	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After the first course of high-dose Ara-C containing consolidation therapy , the patient developed multiple skin lesions on the left foot .
	manualset3
196682	1	416087	7	NULL	NULL	0	NULL	Unitarity triangle	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Unitarity triangle without semileptonic decays .
	manualset3
196683	2	416087	7	NULL	NULL	0	NULL	semileptonic decays	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Unitarity triangle without semileptonic decays .
	manualset3
196684	1	416088	7	NULL	NULL	0	NULL	hysteresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Unless hysteresis is included in the analysis , light NAPL ( LNAPL ) in homogeneous soils can not exist in pools at all , and dense NAPL ( DNAPL ) will not mound on horizontal textural interfaces unless lateral confining boundaries are present .
	manualset3
196685	2	416088	7	NULL	NULL	0	NULL	 analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Unless hysteresis is included in the analysis , light NAPL ( LNAPL ) in homogeneous soils can not exist in pools at all , and dense NAPL ( DNAPL ) will not mound on horizontal textural interfaces unless lateral confining boundaries are present .
	manualset3
196686	3	416088	7	NULL	NULL	0	NULL	light NAPL ( LNAPL )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Unless hysteresis is included in the analysis , light NAPL ( LNAPL ) in homogeneous soils can not exist in pools at all , and dense NAPL ( DNAPL ) will not mound on horizontal textural interfaces unless lateral confining boundaries are present .
	manualset3
196687	4	416088	7	NULL	NULL	0	NULL	homogeneous soils	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Unless hysteresis is included in the analysis , light NAPL ( LNAPL ) in homogeneous soils can not exist in pools at all , and dense NAPL ( DNAPL ) will not mound on horizontal textural interfaces unless lateral confining boundaries are present .
	manualset3
196688	5	416088	7	NULL	NULL	NULL	NULL	 pools	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Unless hysteresis is included in the analysis , light NAPL ( LNAPL ) in homogeneous soils can not exist in pools at all , and dense NAPL ( DNAPL ) will not mound on horizontal textural interfaces unless lateral confining boundaries are present .
	manualset3
196689	6	416088	7	NULL	NULL	0	NULL	dense NAPL ( DNAPL )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Unless hysteresis is included in the analysis , light NAPL ( LNAPL ) in homogeneous soils can not exist in pools at all , and dense NAPL ( DNAPL ) will not mound on horizontal textural interfaces unless lateral confining boundaries are present .
	manualset3
196690	7	416088	7	NULL	NULL	0	NULL	horizontal textural interfaces	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Unless hysteresis is included in the analysis , light NAPL ( LNAPL ) in homogeneous soils can not exist in pools at all , and dense NAPL ( DNAPL ) will not mound on horizontal textural interfaces unless lateral confining boundaries are present .
	manualset3
196691	8	416088	7	NULL	NULL	0	NULL	 lateral confining boundaries 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Unless hysteresis is included in the analysis , light NAPL ( LNAPL ) in homogeneous soils can not exist in pools at all , and dense NAPL ( DNAPL ) will not mound on horizontal textural interfaces unless lateral confining boundaries are present .
	manualset3
196692	1	416089	7	NULL	NULL	0	NULL	clathrin-mediated endocytosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike clathrin-mediated endocytosis , internalization through caveolae is a triggered event that involves complex signaling .
	manualset3
196693	2	416089	7	NULL	NULL	0	NULL	internalization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike clathrin-mediated endocytosis , internalization through caveolae is a triggered event that involves complex signaling .
	manualset3
196694	3	416089	7	NULL	NULL	NULL	NULL	 caveolae	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Unlike clathrin-mediated endocytosis , internalization through caveolae is a triggered event that involves complex signaling .
	manualset3
196695	4	416089	7	NULL	NULL	NULL	NULL	triggered event 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Unlike clathrin-mediated endocytosis , internalization through caveolae is a triggered event that involves complex signaling .
	manualset3
196696	5	416089	7	NULL	NULL	0	NULL	complex signaling	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike clathrin-mediated endocytosis , internalization through caveolae is a triggered event that involves complex signaling .
	manualset3
196697	1	416090	7	NULL	NULL	0	NULL	pancreas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike in pancreas of other animals , the prophospholipase A2 was not detectable in gastric mucosa or juice homogenates treated with diisopropyl fluorophosphate or in column effluents during purification under acidic conditions .
	manualset3
196698	2	416090	7	NULL	NULL	0	NULL	 animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike in pancreas of other animals , the prophospholipase A2 was not detectable in gastric mucosa or juice homogenates treated with diisopropyl fluorophosphate or in column effluents during purification under acidic conditions .
	manualset3
196699	3	416090	7	NULL	NULL	0	NULL	prophospholipase A2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike in pancreas of other animals , the prophospholipase A2 was not detectable in gastric mucosa or juice homogenates treated with diisopropyl fluorophosphate or in column effluents during purification under acidic conditions .
	manualset3
196700	4	416090	7	NULL	NULL	0	NULL	gastric mucosa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike in pancreas of other animals , the prophospholipase A2 was not detectable in gastric mucosa or juice homogenates treated with diisopropyl fluorophosphate or in column effluents during purification under acidic conditions .
	manualset3
196701	5	416090	7	NULL	NULL	0	NULL	juice homogenates	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike in pancreas of other animals , the prophospholipase A2 was not detectable in gastric mucosa or juice homogenates treated with diisopropyl fluorophosphate or in column effluents during purification under acidic conditions .
	manualset3
196702	6	416090	7	NULL	NULL	0	NULL	diisopropyl fluorophosphate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike in pancreas of other animals , the prophospholipase A2 was not detectable in gastric mucosa or juice homogenates treated with diisopropyl fluorophosphate or in column effluents during purification under acidic conditions .
	manualset3
196703	7	416090	7	NULL	NULL	0	NULL	column effluents 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike in pancreas of other animals , the prophospholipase A2 was not detectable in gastric mucosa or juice homogenates treated with diisopropyl fluorophosphate or in column effluents during purification under acidic conditions .
	manualset3
196704	8	416090	7	NULL	NULL	0	NULL	purification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike in pancreas of other animals , the prophospholipase A2 was not detectable in gastric mucosa or juice homogenates treated with diisopropyl fluorophosphate or in column effluents during purification under acidic conditions .
	manualset3
196705	9	416090	7	NULL	NULL	0	NULL	acidic conditions 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike in pancreas of other animals , the prophospholipase A2 was not detectable in gastric mucosa or juice homogenates treated with diisopropyl fluorophosphate or in column effluents during purification under acidic conditions .
	manualset3
196805	1	416091	7	NULL	NULL	0	NULL	approaches	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike previous approaches , our Hamiltonians are not only exactly solvable with exact ground state degeneracy , but also support completely localized quasiparticle excitations , which are ideal for quantum information processing tasks .
	manualset3
196806	2	416091	7	NULL	NULL	0	NULL	Hamiltonians	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike previous approaches , our Hamiltonians are not only exactly solvable with exact ground state degeneracy , but also support completely localized quasiparticle excitations , which are ideal for quantum information processing tasks .
	manualset3
196807	3	416091	7	NULL	NULL	0	NULL	exact ground state degeneracy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike previous approaches , our Hamiltonians are not only exactly solvable with exact ground state degeneracy , but also support completely localized quasiparticle excitations , which are ideal for quantum information processing tasks .
	manualset3
196808	4	416091	7	NULL	NULL	0	NULL	quasiparticle excitations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike previous approaches , our Hamiltonians are not only exactly solvable with exact ground state degeneracy , but also support completely localized quasiparticle excitations , which are ideal for quantum information processing tasks .
	manualset3
196809	5	416091	7	NULL	NULL	0	NULL	quantum information processing tasks	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike previous approaches , our Hamiltonians are not only exactly solvable with exact ground state degeneracy , but also support completely localized quasiparticle excitations , which are ideal for quantum information processing tasks .
	manualset3
196810	1	416092	7	NULL	NULL	0	NULL	absorption phase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike the absorption phase , a statistical difference was not detected between Neupogen and LeukoCIM for clearance ( 18.69 + / -11.83 versus 28.42 + / -12.11 mL/h/kg , P = 0.22 ) .
	manualset3
196811	2	416092	7	NULL	NULL	0	NULL	statistical difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike the absorption phase , a statistical difference was not detected between Neupogen and LeukoCIM for clearance ( 18.69 + / -11.83 versus 28.42 + / -12.11 mL/h/kg , P = 0.22 ) .
	manualset3
196812	3	416092	7	NULL	NULL	0	NULL	Neupogen	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike the absorption phase , a statistical difference was not detected between Neupogen and LeukoCIM for clearance ( 18.69 + / -11.83 versus 28.42 + / -12.11 mL/h/kg , P = 0.22 ) .
	manualset3
196813	4	416092	7	NULL	NULL	0	NULL	LeukoCIM	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike the absorption phase , a statistical difference was not detected between Neupogen and LeukoCIM for clearance ( 18.69 + / -11.83 versus 28.42 + / -12.11 mL/h/kg , P = 0.22 ) .
	manualset3
196814	5	416092	7	NULL	NULL	0	NULL	clearance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike the absorption phase , a statistical difference was not detected between Neupogen and LeukoCIM for clearance ( 18.69 + / -11.83 versus 28.42 + / -12.11 mL/h/kg , P = 0.22 ) .
	manualset3
196815	6	416092	7	NULL	NULL	0	NULL	18.69 + / -11.83	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike the absorption phase , a statistical difference was not detected between Neupogen and LeukoCIM for clearance ( 18.69 + / -11.83 versus 28.42 + / -12.11 mL/h/kg , P = 0.22 ) .
	manualset3
196816	7	416092	7	NULL	NULL	0	NULL	28.42 + / -12.11 mL/h/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike the absorption phase , a statistical difference was not detected between Neupogen and LeukoCIM for clearance ( 18.69 + / -11.83 versus 28.42 + / -12.11 mL/h/kg , P = 0.22 ) .
	manualset3
196817	8	416092	7	NULL	NULL	0	NULL	P = 0.22	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike the absorption phase , a statistical difference was not detected between Neupogen and LeukoCIM for clearance ( 18.69 + / -11.83 versus 28.42 + / -12.11 mL/h/kg , P = 0.22 ) .
	manualset3
196818	1	416093	7	NULL	NULL	0	NULL	 today	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike today , care in the community was a communal activity that ensured a truly public provision for those who could not look after themselves .
	manualset3
196819	2	416093	7	NULL	NULL	0	NULL	care	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike today , care in the community was a communal activity that ensured a truly public provision for those who could not look after themselves .
	manualset3
196820	3	416093	7	NULL	NULL	0	NULL	community	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike today , care in the community was a communal activity that ensured a truly public provision for those who could not look after themselves .
	manualset3
196821	4	416093	7	NULL	NULL	0	NULL	communal activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike today , care in the community was a communal activity that ensured a truly public provision for those who could not look after themselves .
	manualset3
196822	5	416093	7	NULL	NULL	0	NULL	public provision	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike today , care in the community was a communal activity that ensured a truly public provision for those who could not look after themselves .
	manualset3
196823	1	416094	7	NULL	NULL	0	NULL	wild-type TBEV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike wild-type TBEV , vTBE ( ME ) / DEN4 did not cause encephalitis when adult mice were inoculated by a peripheral route .
	manualset3
196824	2	416094	7	NULL	NULL	0	NULL	 vTBE ( ME )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike wild-type TBEV , vTBE ( ME ) / DEN4 did not cause encephalitis when adult mice were inoculated by a peripheral route .
	manualset3
196825	3	416094	7	NULL	NULL	0	NULL	DEN4	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike wild-type TBEV , vTBE ( ME ) / DEN4 did not cause encephalitis when adult mice were inoculated by a peripheral route .
	manualset3
196826	4	416094	7	NULL	NULL	0	NULL	encephalitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike wild-type TBEV , vTBE ( ME ) / DEN4 did not cause encephalitis when adult mice were inoculated by a peripheral route .
	manualset3
196827	5	416094	7	NULL	NULL	0	NULL	adult mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike wild-type TBEV , vTBE ( ME ) / DEN4 did not cause encephalitis when adult mice were inoculated by a peripheral route .
	manualset3
196828	6	416094	7	NULL	NULL	0	NULL	peripheral route	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlike wild-type TBEV , vTBE ( ME ) / DEN4 did not cause encephalitis when adult mice were inoculated by a peripheral route .
	manualset3
196829	1	416095	7	NULL	NULL	0	NULL	five-month intervention period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After the five-month intervention period , 34 % of participants reported use of device in the preceding week and 13 % reported consistent use .
	manualset3
196830	2	416095	7	NULL	NULL	0	NULL	34 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After the five-month intervention period , 34 % of participants reported use of device in the preceding week and 13 % reported consistent use .
	manualset3
196831	3	416095	7	NULL	NULL	0	NULL	participants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	After the five-month intervention period , 34 % of participants reported use of device in the preceding week and 13 % reported consistent use .
	manualset3
196832	4	416095	7	NULL	NULL	0	NULL	device	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	After the five-month intervention period , 34 % of participants reported use of device in the preceding week and 13 % reported consistent use .
	manualset3
196833	5	416095	7	NULL	NULL	0	NULL	preceding week 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After the five-month intervention period , 34 % of participants reported use of device in the preceding week and 13 % reported consistent use .
	manualset3
196834	6	416095	7	NULL	NULL	0	NULL	13 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After the five-month intervention period , 34 % of participants reported use of device in the preceding week and 13 % reported consistent use .
	manualset3
196835	1	416096	7	NULL	NULL	0	NULL	Unlock the door	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlock the door on youth problems : the adolescent from eleven to sixteen years .
	manualset3
196836	2	416096	7	NULL	NULL	0	NULL	youth problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlock the door on youth problems : the adolescent from eleven to sixteen years .
	manualset3
196837	3	416096	7	NULL	NULL	0	NULL	 adolescent 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlock the door on youth problems : the adolescent from eleven to sixteen years .
	manualset3
196838	4	416096	7	NULL	NULL	0	NULL	eleven years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlock the door on youth problems : the adolescent from eleven to sixteen years .
	manualset3
196839	5	416096	7	NULL	NULL	0	NULL	sixteen years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Unlock the door on youth problems : the adolescent from eleven to sixteen years .
	manualset3
196840	1	416097	7	NULL	NULL	0	NULL	Unrecognised articular penetration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Unrecognised articular penetration and damage during surgery were confirmed in four .
	manualset3
196841	2	416097	7	NULL	NULL	0	NULL	damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Unrecognised articular penetration and damage during surgery were confirmed in four .
	manualset3
196842	3	416097	7	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Unrecognised articular penetration and damage during surgery were confirmed in four .
	manualset3
196843	4	416097	7	NULL	NULL	0	NULL	four	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Unrecognised articular penetration and damage during surgery were confirmed in four .
	manualset3
196844	1	416098	7	NULL	NULL	0	NULL	Unrelated BMT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Unrelated BMT should be considered as a treatment option for patients with high-risk NHL without an HLA-matched related donor .
	manualset3
196845	2	416098	7	NULL	NULL	0	NULL	 treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Unrelated BMT should be considered as a treatment option for patients with high-risk NHL without an HLA-matched related donor .
	manualset3
196846	3	416098	7	NULL	NULL	0	NULL	 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Unrelated BMT should be considered as a treatment option for patients with high-risk NHL without an HLA-matched related donor .
	manualset3
196847	4	416098	7	NULL	NULL	0	NULL	 high-risk NHL 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Unrelated BMT should be considered as a treatment option for patients with high-risk NHL without an HLA-matched related donor .
	manualset3
196848	5	416098	7	NULL	NULL	NULL	NULL	HLA-matched related donor	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Unrelated BMT should be considered as a treatment option for patients with high-risk NHL without an HLA-matched related donor .
	manualset3
196849	1	416099	7	NULL	NULL	0	NULL	Unstable clones	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Unstable clones excreting L-lysine into their growth medium are obtained at a very high frequency following UV irradiation in both haploid and diploid strains of Saccharomycopsis lipolytica , provided they carry a mutation affecting the first enzyme of the lysine pathway and confering resistance to end product inhibition .
	manualset3
196850	2	416099	7	NULL	NULL	0	NULL	L-lysine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Unstable clones excreting L-lysine into their growth medium are obtained at a very high frequency following UV irradiation in both haploid and diploid strains of Saccharomycopsis lipolytica , provided they carry a mutation affecting the first enzyme of the lysine pathway and confering resistance to end product inhibition .
	manualset3
196851	3	416099	7	NULL	NULL	0	NULL	growth medium	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Unstable clones excreting L-lysine into their growth medium are obtained at a very high frequency following UV irradiation in both haploid and diploid strains of Saccharomycopsis lipolytica , provided they carry a mutation affecting the first enzyme of the lysine pathway and confering resistance to end product inhibition .
	manualset3
196852	4	416099	7	NULL	NULL	0	NULL	high frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Unstable clones excreting L-lysine into their growth medium are obtained at a very high frequency following UV irradiation in both haploid and diploid strains of Saccharomycopsis lipolytica , provided they carry a mutation affecting the first enzyme of the lysine pathway and confering resistance to end product inhibition .
	manualset3
196853	5	416099	7	NULL	NULL	0	NULL	UV irradiation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Unstable clones excreting L-lysine into their growth medium are obtained at a very high frequency following UV irradiation in both haploid and diploid strains of Saccharomycopsis lipolytica , provided they carry a mutation affecting the first enzyme of the lysine pathway and confering resistance to end product inhibition .
	manualset3
196854	6	416099	7	NULL	NULL	0	NULL	haploid strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Unstable clones excreting L-lysine into their growth medium are obtained at a very high frequency following UV irradiation in both haploid and diploid strains of Saccharomycopsis lipolytica , provided they carry a mutation affecting the first enzyme of the lysine pathway and confering resistance to end product inhibition .
	manualset3
196855	7	416099	7	NULL	NULL	0	NULL	diploid strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Unstable clones excreting L-lysine into their growth medium are obtained at a very high frequency following UV irradiation in both haploid and diploid strains of Saccharomycopsis lipolytica , provided they carry a mutation affecting the first enzyme of the lysine pathway and confering resistance to end product inhibition .
	manualset3
196856	8	416099	7	NULL	NULL	0	NULL	Saccharomycopsis lipolytica 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Unstable clones excreting L-lysine into their growth medium are obtained at a very high frequency following UV irradiation in both haploid and diploid strains of Saccharomycopsis lipolytica , provided they carry a mutation affecting the first enzyme of the lysine pathway and confering resistance to end product inhibition .
	manualset3
196857	9	416099	7	NULL	NULL	0	NULL	mutation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unstable clones excreting L-lysine into their growth medium are obtained at a very high frequency following UV irradiation in both haploid and diploid strains of Saccharomycopsis lipolytica , provided they carry a mutation affecting the first enzyme of the lysine pathway and confering resistance to end product inhibition .
	manualset3
196858	10	416099	7	NULL	NULL	0	NULL	first enzyme	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Unstable clones excreting L-lysine into their growth medium are obtained at a very high frequency following UV irradiation in both haploid and diploid strains of Saccharomycopsis lipolytica , provided they carry a mutation affecting the first enzyme of the lysine pathway and confering resistance to end product inhibition .
	manualset3
196859	11	416099	7	NULL	NULL	0	NULL	lysine pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unstable clones excreting L-lysine into their growth medium are obtained at a very high frequency following UV irradiation in both haploid and diploid strains of Saccharomycopsis lipolytica , provided they carry a mutation affecting the first enzyme of the lysine pathway and confering resistance to end product inhibition .
	manualset3
196860	12	416099	7	NULL	NULL	0	NULL	resistance	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unstable clones excreting L-lysine into their growth medium are obtained at a very high frequency following UV irradiation in both haploid and diploid strains of Saccharomycopsis lipolytica , provided they carry a mutation affecting the first enzyme of the lysine pathway and confering resistance to end product inhibition .
	manualset3
196861	13	416099	7	NULL	NULL	0	NULL	product inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unstable clones excreting L-lysine into their growth medium are obtained at a very high frequency following UV irradiation in both haploid and diploid strains of Saccharomycopsis lipolytica , provided they carry a mutation affecting the first enzyme of the lysine pathway and confering resistance to end product inhibition .
	manualset3
196862	1	416100	7	NULL	NULL	0	NULL	Unsupervised clustering 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unsupervised clustering in mRNA expression profiles .
	manualset3
196863	2	416100	7	NULL	NULL	0	NULL	mRNA expression profiles	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unsupervised clustering in mRNA expression profiles .
	manualset3
196864	1	416101	7	NULL	NULL	0	NULL	2008	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Until 2008 poliomyelitis was controlled in Romania by predominantly using Oral Poliovirus Vaccine Sabin ( OPV ) ; the alternative vaccination schedule ( IPV formalin Inactivated Poliovirus Vaccine/OPV ) will be implemented starting September 2008 .
	manualset3
196865	2	416101	7	NULL	NULL	0	NULL	poliomyelitis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Until 2008 poliomyelitis was controlled in Romania by predominantly using Oral Poliovirus Vaccine Sabin ( OPV ) ; the alternative vaccination schedule ( IPV formalin Inactivated Poliovirus Vaccine/OPV ) will be implemented starting September 2008 .
	manualset3
196866	3	416101	7	NULL	NULL	0	NULL	Romania	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Until 2008 poliomyelitis was controlled in Romania by predominantly using Oral Poliovirus Vaccine Sabin ( OPV ) ; the alternative vaccination schedule ( IPV formalin Inactivated Poliovirus Vaccine/OPV ) will be implemented starting September 2008 .
	manualset3
196867	4	416101	7	NULL	NULL	NULL	NULL	Oral Poliovirus Vaccine Sabin ( OPV )	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Until 2008 poliomyelitis was controlled in Romania by predominantly using Oral Poliovirus Vaccine Sabin ( OPV ) ; the alternative vaccination schedule ( IPV formalin Inactivated Poliovirus Vaccine/OPV ) will be implemented starting September 2008 .
	manualset3
196868	5	416101	7	NULL	NULL	0	NULL	alternative vaccination schedule	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Until 2008 poliomyelitis was controlled in Romania by predominantly using Oral Poliovirus Vaccine Sabin ( OPV ) ; the alternative vaccination schedule ( IPV formalin Inactivated Poliovirus Vaccine/OPV ) will be implemented starting September 2008 .
	manualset3
196869	6	416101	7	NULL	NULL	0	NULL	IPV formalin Inactivated Poliovirus Vaccine/OPV )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Until 2008 poliomyelitis was controlled in Romania by predominantly using Oral Poliovirus Vaccine Sabin ( OPV ) ; the alternative vaccination schedule ( IPV formalin Inactivated Poliovirus Vaccine/OPV ) will be implemented starting September 2008 .
	manualset3
196870	7	416101	7	NULL	NULL	0	NULL	September 2008	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Until 2008 poliomyelitis was controlled in Romania by predominantly using Oral Poliovirus Vaccine Sabin ( OPV ) ; the alternative vaccination schedule ( IPV formalin Inactivated Poliovirus Vaccine/OPV ) will be implemented starting September 2008 .
	manualset3
196871	1	416102	7	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Until growth has come to an end , continuous follow-up is necessary for early recognizing late contractures .
	manualset3
196872	2	416102	7	NULL	NULL	0	NULL	continuous follow-up	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Until growth has come to an end , continuous follow-up is necessary for early recognizing late contractures .
	manualset3
196873	3	416102	7	NULL	NULL	0	NULL	early recognizing late contractures 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Until growth has come to an end , continuous follow-up is necessary for early recognizing late contractures .
	manualset3
196874	1	416103	7	NULL	NULL	0	NULL	 information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Until now information about the influence of puberty on gingival tissue responses to Ni-Ti alloy have n't been available .
	manualset3
196875	2	416103	7	NULL	NULL	0	NULL	influence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Until now information about the influence of puberty on gingival tissue responses to Ni-Ti alloy have n't been available .
	manualset3
196876	3	416103	7	NULL	NULL	0	NULL	 puberty	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Until now information about the influence of puberty on gingival tissue responses to Ni-Ti alloy have n't been available .
	manualset3
196877	4	416103	7	NULL	NULL	NULL	NULL	gingival tissue responses	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Until now information about the influence of puberty on gingival tissue responses to Ni-Ti alloy have n't been available .
	manualset3
196878	5	416103	7	NULL	NULL	0	NULL	Ni-Ti alloy	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Until now information about the influence of puberty on gingival tissue responses to Ni-Ti alloy have n't been available .
	manualset3
196879	1	416104	7	NULL	NULL	0	NULL	 research 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Until such research appears , caution is urged to those who would attempt to use this instrument in clinical situations .
	manualset3
196880	2	416104	7	NULL	NULL	0	NULL	caution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Until such research appears , caution is urged to those who would attempt to use this instrument in clinical situations .
	manualset3
196881	3	416104	7	NULL	NULL	0	NULL	instrument	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Until such research appears , caution is urged to those who would attempt to use this instrument in clinical situations .
	manualset3
196882	4	416104	7	NULL	NULL	0	NULL	 clinical situations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Until such research appears , caution is urged to those who would attempt to use this instrument in clinical situations .
	manualset3
196883	1	416105	7	NULL	NULL	0	NULL	early 1970s	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Until the early 1970s , the guidelines for fluid ingestion during exercise were not to drink and are consistent with this interpretation .
	manualset3
196884	2	416105	7	NULL	NULL	0	NULL	guidelines 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Until the early 1970s , the guidelines for fluid ingestion during exercise were not to drink and are consistent with this interpretation .
	manualset3
196885	3	416105	7	NULL	NULL	0	NULL	fluid ingestion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Until the early 1970s , the guidelines for fluid ingestion during exercise were not to drink and are consistent with this interpretation .
	manualset3
196886	4	416105	7	NULL	NULL	0	NULL	exercise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Until the early 1970s , the guidelines for fluid ingestion during exercise were not to drink and are consistent with this interpretation .
	manualset3
196887	5	416105	7	NULL	NULL	0	NULL	interpretation	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Until the early 1970s , the guidelines for fluid ingestion during exercise were not to drink and are consistent with this interpretation .
	manualset3
196888	1	416106	7	NULL	NULL	NULL	NULL	Untrained men participants	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Untrained men and women participants were separated into 4 groups : group A ( n = 17 , 71.4 + / - 4.6 years ) performed 2 sets of 15 repetitions maximum ( RM ) , group B ( n = 13 , 71.5 + / - 5.2 years ) performed 3 sets of 9 RM , group C ( n = 17 , 69.4 + / - 4.4 years ) performed 4 sets of 6 RM , group D ( n = 14 , 72.3 + / - 5.9 years ) served as controls .
	manualset3
196889	2	416106	7	NULL	NULL	NULL	NULL	Untrained women participants	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Untrained men and women participants were separated into 4 groups : group A ( n = 17 , 71.4 + / - 4.6 years ) performed 2 sets of 15 repetitions maximum ( RM ) , group B ( n = 13 , 71.5 + / - 5.2 years ) performed 3 sets of 9 RM , group C ( n = 17 , 69.4 + / - 4.4 years ) performed 4 sets of 6 RM , group D ( n = 14 , 72.3 + / - 5.9 years ) served as controls .
	manualset3
196890	3	416106	7	NULL	NULL	0	NULL	4 groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Untrained men and women participants were separated into 4 groups : group A ( n = 17 , 71.4 + / - 4.6 years ) performed 2 sets of 15 repetitions maximum ( RM ) , group B ( n = 13 , 71.5 + / - 5.2 years ) performed 3 sets of 9 RM , group C ( n = 17 , 69.4 + / - 4.4 years ) performed 4 sets of 6 RM , group D ( n = 14 , 72.3 + / - 5.9 years ) served as controls .
	manualset3
196891	4	416106	7	NULL	NULL	0	NULL	group A	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Untrained men and women participants were separated into 4 groups : group A ( n = 17 , 71.4 + / - 4.6 years ) performed 2 sets of 15 repetitions maximum ( RM ) , group B ( n = 13 , 71.5 + / - 5.2 years ) performed 3 sets of 9 RM , group C ( n = 17 , 69.4 + / - 4.4 years ) performed 4 sets of 6 RM , group D ( n = 14 , 72.3 + / - 5.9 years ) served as controls .
	manualset3
196892	5	416106	7	NULL	NULL	0	NULL	( n = 17 , 71.4 + / - 4.6 years )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Untrained men and women participants were separated into 4 groups : group A ( n = 17 , 71.4 + / - 4.6 years ) performed 2 sets of 15 repetitions maximum ( RM ) , group B ( n = 13 , 71.5 + / - 5.2 years ) performed 3 sets of 9 RM , group C ( n = 17 , 69.4 + / - 4.4 years ) performed 4 sets of 6 RM , group D ( n = 14 , 72.3 + / - 5.9 years ) served as controls .
	manualset3
196893	6	416106	7	NULL	NULL	0	NULL	2 sets	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Untrained men and women participants were separated into 4 groups : group A ( n = 17 , 71.4 + / - 4.6 years ) performed 2 sets of 15 repetitions maximum ( RM ) , group B ( n = 13 , 71.5 + / - 5.2 years ) performed 3 sets of 9 RM , group C ( n = 17 , 69.4 + / - 4.4 years ) performed 4 sets of 6 RM , group D ( n = 14 , 72.3 + / - 5.9 years ) served as controls .
	manualset3
196894	7	416106	7	NULL	NULL	0	NULL	15 repetitions maximum ( RM )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Untrained men and women participants were separated into 4 groups : group A ( n = 17 , 71.4 + / - 4.6 years ) performed 2 sets of 15 repetitions maximum ( RM ) , group B ( n = 13 , 71.5 + / - 5.2 years ) performed 3 sets of 9 RM , group C ( n = 17 , 69.4 + / - 4.4 years ) performed 4 sets of 6 RM , group D ( n = 14 , 72.3 + / - 5.9 years ) served as controls .
	manualset3
196895	8	416106	7	NULL	NULL	0	NULL	group B	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Untrained men and women participants were separated into 4 groups : group A ( n = 17 , 71.4 + / - 4.6 years ) performed 2 sets of 15 repetitions maximum ( RM ) , group B ( n = 13 , 71.5 + / - 5.2 years ) performed 3 sets of 9 RM , group C ( n = 17 , 69.4 + / - 4.4 years ) performed 4 sets of 6 RM , group D ( n = 14 , 72.3 + / - 5.9 years ) served as controls .
	manualset3
196896	9	416106	7	NULL	NULL	0	NULL	( n = 13 , 71.5 + / - 5.2 years )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Untrained men and women participants were separated into 4 groups : group A ( n = 17 , 71.4 + / - 4.6 years ) performed 2 sets of 15 repetitions maximum ( RM ) , group B ( n = 13 , 71.5 + / - 5.2 years ) performed 3 sets of 9 RM , group C ( n = 17 , 69.4 + / - 4.4 years ) performed 4 sets of 6 RM , group D ( n = 14 , 72.3 + / - 5.9 years ) served as controls .
	manualset3
196897	10	416106	7	NULL	NULL	0	NULL	3 sets 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Untrained men and women participants were separated into 4 groups : group A ( n = 17 , 71.4 + / - 4.6 years ) performed 2 sets of 15 repetitions maximum ( RM ) , group B ( n = 13 , 71.5 + / - 5.2 years ) performed 3 sets of 9 RM , group C ( n = 17 , 69.4 + / - 4.4 years ) performed 4 sets of 6 RM , group D ( n = 14 , 72.3 + / - 5.9 years ) served as controls .
	manualset3
196898	11	416106	7	NULL	NULL	0	NULL	 9 RM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Untrained men and women participants were separated into 4 groups : group A ( n = 17 , 71.4 + / - 4.6 years ) performed 2 sets of 15 repetitions maximum ( RM ) , group B ( n = 13 , 71.5 + / - 5.2 years ) performed 3 sets of 9 RM , group C ( n = 17 , 69.4 + / - 4.4 years ) performed 4 sets of 6 RM , group D ( n = 14 , 72.3 + / - 5.9 years ) served as controls .
	manualset3
196899	12	416106	7	NULL	NULL	0	NULL	group C	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Untrained men and women participants were separated into 4 groups : group A ( n = 17 , 71.4 + / - 4.6 years ) performed 2 sets of 15 repetitions maximum ( RM ) , group B ( n = 13 , 71.5 + / - 5.2 years ) performed 3 sets of 9 RM , group C ( n = 17 , 69.4 + / - 4.4 years ) performed 4 sets of 6 RM , group D ( n = 14 , 72.3 + / - 5.9 years ) served as controls .
	manualset3
196900	13	416106	7	NULL	NULL	0	NULL	( n = 17 , 69.4 + / - 4.4 years )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Untrained men and women participants were separated into 4 groups : group A ( n = 17 , 71.4 + / - 4.6 years ) performed 2 sets of 15 repetitions maximum ( RM ) , group B ( n = 13 , 71.5 + / - 5.2 years ) performed 3 sets of 9 RM , group C ( n = 17 , 69.4 + / - 4.4 years ) performed 4 sets of 6 RM , group D ( n = 14 , 72.3 + / - 5.9 years ) served as controls .
	manualset3
196901	14	416106	7	NULL	NULL	0	NULL	4 sets	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Untrained men and women participants were separated into 4 groups : group A ( n = 17 , 71.4 + / - 4.6 years ) performed 2 sets of 15 repetitions maximum ( RM ) , group B ( n = 13 , 71.5 + / - 5.2 years ) performed 3 sets of 9 RM , group C ( n = 17 , 69.4 + / - 4.4 years ) performed 4 sets of 6 RM , group D ( n = 14 , 72.3 + / - 5.9 years ) served as controls .
	manualset3
196902	15	416106	7	NULL	NULL	0	NULL	6 RM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Untrained men and women participants were separated into 4 groups : group A ( n = 17 , 71.4 + / - 4.6 years ) performed 2 sets of 15 repetitions maximum ( RM ) , group B ( n = 13 , 71.5 + / - 5.2 years ) performed 3 sets of 9 RM , group C ( n = 17 , 69.4 + / - 4.4 years ) performed 4 sets of 6 RM , group D ( n = 14 , 72.3 + / - 5.9 years ) served as controls .
	manualset3
196903	16	416106	7	NULL	NULL	0	NULL	 group D	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Untrained men and women participants were separated into 4 groups : group A ( n = 17 , 71.4 + / - 4.6 years ) performed 2 sets of 15 repetitions maximum ( RM ) , group B ( n = 13 , 71.5 + / - 5.2 years ) performed 3 sets of 9 RM , group C ( n = 17 , 69.4 + / - 4.4 years ) performed 4 sets of 6 RM , group D ( n = 14 , 72.3 + / - 5.9 years ) served as controls .
	manualset3
196904	17	416106	7	NULL	NULL	0	NULL	( n = 14 , 72.3 + / - 5.9 years )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Untrained men and women participants were separated into 4 groups : group A ( n = 17 , 71.4 + / - 4.6 years ) performed 2 sets of 15 repetitions maximum ( RM ) , group B ( n = 13 , 71.5 + / - 5.2 years ) performed 3 sets of 9 RM , group C ( n = 17 , 69.4 + / - 4.4 years ) performed 4 sets of 6 RM , group D ( n = 14 , 72.3 + / - 5.9 years ) served as controls .
	manualset3
196905	18	416106	7	NULL	NULL	0	NULL	controls	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Untrained men and women participants were separated into 4 groups : group A ( n = 17 , 71.4 + / - 4.6 years ) performed 2 sets of 15 repetitions maximum ( RM ) , group B ( n = 13 , 71.5 + / - 5.2 years ) performed 3 sets of 9 RM , group C ( n = 17 , 69.4 + / - 4.4 years ) performed 4 sets of 6 RM , group D ( n = 14 , 72.3 + / - 5.9 years ) served as controls .
	manualset3
196906	1	416107	7	NULL	NULL	0	NULL	Up-regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Up-regulation of galanin and corticotropin-releasing hormone mRNAs in the key hypothalamic and amygdaloid nuclei in a mouse model of visceral pain .
	manualset3
196907	2	416107	7	NULL	NULL	0	NULL	galanin mRNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Up-regulation of galanin and corticotropin-releasing hormone mRNAs in the key hypothalamic and amygdaloid nuclei in a mouse model of visceral pain .
	manualset3
196908	3	416107	7	NULL	NULL	0	NULL	corticotropin-releasing hormone mRNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Up-regulation of galanin and corticotropin-releasing hormone mRNAs in the key hypothalamic and amygdaloid nuclei in a mouse model of visceral pain .
	manualset3
196909	4	416107	7	NULL	NULL	0	NULL	hypothalamic nuclei	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Up-regulation of galanin and corticotropin-releasing hormone mRNAs in the key hypothalamic and amygdaloid nuclei in a mouse model of visceral pain .
	manualset3
196910	5	416107	7	NULL	NULL	0	NULL	amygdaloid nuclei	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Up-regulation of galanin and corticotropin-releasing hormone mRNAs in the key hypothalamic and amygdaloid nuclei in a mouse model of visceral pain .
	manualset3
196911	6	416107	7	NULL	NULL	0	NULL	mouse model 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Up-regulation of galanin and corticotropin-releasing hormone mRNAs in the key hypothalamic and amygdaloid nuclei in a mouse model of visceral pain .
	manualset3
196912	7	416107	7	NULL	NULL	0	NULL	visceral pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Up-regulation of galanin and corticotropin-releasing hormone mRNAs in the key hypothalamic and amygdaloid nuclei in a mouse model of visceral pain .
	manualset3
196913	1	416108	7	NULL	NULL	0	NULL	500-fold enrichment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Up to 500-fold enrichment of analytes could be obtained under the optimized conditions ( donor solution : 0.1 M sodium hydroxide solution with 20 % sodium chloride and 2 % acetone ; organic phase : di-n-hexyl ether ; acceptor solution : 0.5 M hydrochloric acid and 500 mM 18-crown-6 ether ; extraction time of 30 min ; stirring at 1 , 000 rev. / min ) .
	manualset3
196914	2	416108	7	NULL	NULL	0	NULL	analytes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Up to 500-fold enrichment of analytes could be obtained under the optimized conditions ( donor solution : 0.1 M sodium hydroxide solution with 20 % sodium chloride and 2 % acetone ; organic phase : di-n-hexyl ether ; acceptor solution : 0.5 M hydrochloric acid and 500 mM 18-crown-6 ether ; extraction time of 30 min ; stirring at 1 , 000 rev. / min ) .
	manualset3
196915	3	416108	7	NULL	NULL	0	NULL	optimized conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Up to 500-fold enrichment of analytes could be obtained under the optimized conditions ( donor solution : 0.1 M sodium hydroxide solution with 20 % sodium chloride and 2 % acetone ; organic phase : di-n-hexyl ether ; acceptor solution : 0.5 M hydrochloric acid and 500 mM 18-crown-6 ether ; extraction time of 30 min ; stirring at 1 , 000 rev. / min ) .
	manualset3
196916	4	416108	7	NULL	NULL	0	NULL	donor solution 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Up to 500-fold enrichment of analytes could be obtained under the optimized conditions ( donor solution : 0.1 M sodium hydroxide solution with 20 % sodium chloride and 2 % acetone ; organic phase : di-n-hexyl ether ; acceptor solution : 0.5 M hydrochloric acid and 500 mM 18-crown-6 ether ; extraction time of 30 min ; stirring at 1 , 000 rev. / min ) .
	manualset3
196917	5	416108	7	NULL	NULL	0	NULL	0.1 M sodium hydroxide solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Up to 500-fold enrichment of analytes could be obtained under the optimized conditions ( donor solution : 0.1 M sodium hydroxide solution with 20 % sodium chloride and 2 % acetone ; organic phase : di-n-hexyl ether ; acceptor solution : 0.5 M hydrochloric acid and 500 mM 18-crown-6 ether ; extraction time of 30 min ; stirring at 1 , 000 rev. / min ) .
	manualset3
196918	6	416108	7	NULL	NULL	0	NULL	20 % sodium chloride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Up to 500-fold enrichment of analytes could be obtained under the optimized conditions ( donor solution : 0.1 M sodium hydroxide solution with 20 % sodium chloride and 2 % acetone ; organic phase : di-n-hexyl ether ; acceptor solution : 0.5 M hydrochloric acid and 500 mM 18-crown-6 ether ; extraction time of 30 min ; stirring at 1 , 000 rev. / min ) .
	manualset3
196919	7	416108	7	NULL	NULL	0	NULL	2 % acetone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Up to 500-fold enrichment of analytes could be obtained under the optimized conditions ( donor solution : 0.1 M sodium hydroxide solution with 20 % sodium chloride and 2 % acetone ; organic phase : di-n-hexyl ether ; acceptor solution : 0.5 M hydrochloric acid and 500 mM 18-crown-6 ether ; extraction time of 30 min ; stirring at 1 , 000 rev. / min ) .
	manualset3
196920	8	416108	7	NULL	NULL	0	NULL	organic phase	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Up to 500-fold enrichment of analytes could be obtained under the optimized conditions ( donor solution : 0.1 M sodium hydroxide solution with 20 % sodium chloride and 2 % acetone ; organic phase : di-n-hexyl ether ; acceptor solution : 0.5 M hydrochloric acid and 500 mM 18-crown-6 ether ; extraction time of 30 min ; stirring at 1 , 000 rev. / min ) .
	manualset3
196921	9	416108	7	NULL	NULL	0	NULL	di-n-hexyl ether	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Up to 500-fold enrichment of analytes could be obtained under the optimized conditions ( donor solution : 0.1 M sodium hydroxide solution with 20 % sodium chloride and 2 % acetone ; organic phase : di-n-hexyl ether ; acceptor solution : 0.5 M hydrochloric acid and 500 mM 18-crown-6 ether ; extraction time of 30 min ; stirring at 1 , 000 rev. / min ) .
	manualset3
196922	10	416108	7	NULL	NULL	0	NULL	acceptor solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Up to 500-fold enrichment of analytes could be obtained under the optimized conditions ( donor solution : 0.1 M sodium hydroxide solution with 20 % sodium chloride and 2 % acetone ; organic phase : di-n-hexyl ether ; acceptor solution : 0.5 M hydrochloric acid and 500 mM 18-crown-6 ether ; extraction time of 30 min ; stirring at 1 , 000 rev. / min ) .
	manualset3
196923	11	416108	7	NULL	NULL	0	NULL	0.5 M hydrochloric acid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Up to 500-fold enrichment of analytes could be obtained under the optimized conditions ( donor solution : 0.1 M sodium hydroxide solution with 20 % sodium chloride and 2 % acetone ; organic phase : di-n-hexyl ether ; acceptor solution : 0.5 M hydrochloric acid and 500 mM 18-crown-6 ether ; extraction time of 30 min ; stirring at 1 , 000 rev. / min ) .
	manualset3
196924	12	416108	7	NULL	NULL	0	NULL	500 mM 18-crown-6 ether	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Up to 500-fold enrichment of analytes could be obtained under the optimized conditions ( donor solution : 0.1 M sodium hydroxide solution with 20 % sodium chloride and 2 % acetone ; organic phase : di-n-hexyl ether ; acceptor solution : 0.5 M hydrochloric acid and 500 mM 18-crown-6 ether ; extraction time of 30 min ; stirring at 1 , 000 rev. / min ) .
	manualset3
196925	13	416108	7	NULL	NULL	0	NULL	extraction time	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Up to 500-fold enrichment of analytes could be obtained under the optimized conditions ( donor solution : 0.1 M sodium hydroxide solution with 20 % sodium chloride and 2 % acetone ; organic phase : di-n-hexyl ether ; acceptor solution : 0.5 M hydrochloric acid and 500 mM 18-crown-6 ether ; extraction time of 30 min ; stirring at 1 , 000 rev. / min ) .
	manualset3
196926	14	416108	7	NULL	NULL	0	NULL	30 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Up to 500-fold enrichment of analytes could be obtained under the optimized conditions ( donor solution : 0.1 M sodium hydroxide solution with 20 % sodium chloride and 2 % acetone ; organic phase : di-n-hexyl ether ; acceptor solution : 0.5 M hydrochloric acid and 500 mM 18-crown-6 ether ; extraction time of 30 min ; stirring at 1 , 000 rev. / min ) .
	manualset3
196927	15	416108	7	NULL	NULL	0	NULL	1 , 000 rev. / min	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Up to 500-fold enrichment of analytes could be obtained under the optimized conditions ( donor solution : 0.1 M sodium hydroxide solution with 20 % sodium chloride and 2 % acetone ; organic phase : di-n-hexyl ether ; acceptor solution : 0.5 M hydrochloric acid and 500 mM 18-crown-6 ether ; extraction time of 30 min ; stirring at 1 , 000 rev. / min ) .
	manualset3
196928	1	416109	7	NULL	NULL	0	NULL	public officials	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Up to now , public officials have shown a clear reluctance to intervene in sprawl areas despite good knowledge of their location .
	manualset3
196929	2	416109	7	NULL	NULL	NULL	NULL	sprawl areas	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Up to now , public officials have shown a clear reluctance to intervene in sprawl areas despite good knowledge of their location .
	manualset3
196930	3	416109	7	NULL	NULL	0	NULL	 good knowledge	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Up to now , public officials have shown a clear reluctance to intervene in sprawl areas despite good knowledge of their location .
	manualset3
196931	4	416109	7	NULL	NULL	NULL	NULL	location	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Up to now , public officials have shown a clear reluctance to intervene in sprawl areas despite good knowledge of their location .
	manualset3
198537	5	416109	7	NULL	NULL	0	NULL	clear reluctance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Up to now , public officials have shown a clear reluctance to intervene in sprawl areas despite good knowledge of their location .
	manualset3
196932	1	416110	7	NULL	NULL	0	NULL	no data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Up to now , there are no data available on whether the fluoride ( F - ) component of these products affects the bactericidal activity of salivary polymorpho-nuclear leucocytes , which are involved in the protection of the oral mucosa against infection .
	manualset3
196933	2	416110	7	NULL	NULL	0	NULL	fluoride ( F - ) component	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Up to now , there are no data available on whether the fluoride ( F - ) component of these products affects the bactericidal activity of salivary polymorpho-nuclear leucocytes , which are involved in the protection of the oral mucosa against infection .
	manualset3
196934	3	416110	7	NULL	NULL	0	NULL	products	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Up to now , there are no data available on whether the fluoride ( F - ) component of these products affects the bactericidal activity of salivary polymorpho-nuclear leucocytes , which are involved in the protection of the oral mucosa against infection .
	manualset3
196935	4	416110	7	NULL	NULL	0	NULL	bactericidal activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Up to now , there are no data available on whether the fluoride ( F - ) component of these products affects the bactericidal activity of salivary polymorpho-nuclear leucocytes , which are involved in the protection of the oral mucosa against infection .
	manualset3
196936	5	416110	7	NULL	NULL	0	NULL	salivary polymorpho-nuclear leucocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Up to now , there are no data available on whether the fluoride ( F - ) component of these products affects the bactericidal activity of salivary polymorpho-nuclear leucocytes , which are involved in the protection of the oral mucosa against infection .
	manualset3
196937	6	416110	7	NULL	NULL	0	NULL	protection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Up to now , there are no data available on whether the fluoride ( F - ) component of these products affects the bactericidal activity of salivary polymorpho-nuclear leucocytes , which are involved in the protection of the oral mucosa against infection .
	manualset3
196938	7	416110	7	NULL	NULL	0	NULL	oral mucosa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Up to now , there are no data available on whether the fluoride ( F - ) component of these products affects the bactericidal activity of salivary polymorpho-nuclear leucocytes , which are involved in the protection of the oral mucosa against infection .
	manualset3
196939	8	416110	7	NULL	NULL	0	NULL	 infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Up to now , there are no data available on whether the fluoride ( F - ) component of these products affects the bactericidal activity of salivary polymorpho-nuclear leucocytes , which are involved in the protection of the oral mucosa against infection .
	manualset3
196940	1	416111	7	NULL	NULL	0	NULL	parturition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After the parturition , the newborn had to be resuscitated .
	manualset3
196941	2	416111	7	NULL	NULL	0	NULL	newborn	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	After the parturition , the newborn had to be resuscitated .
	manualset3
196942	1	416112	7	NULL	NULL	0	NULL	Updated tables`	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Updated tables of vibrational energy levels , molecular constants , band origins , and intensities for carbon dioxide in the infrared region of the spectrum are presented .
	manualset3
196943	2	416112	7	NULL	NULL	NULL	NULL	vibrational energy levels 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Updated tables of vibrational energy levels , molecular constants , band origins , and intensities for carbon dioxide in the infrared region of the spectrum are presented .
	manualset3
196944	3	416112	7	NULL	NULL	0	NULL	molecular constants	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Updated tables of vibrational energy levels , molecular constants , band origins , and intensities for carbon dioxide in the infrared region of the spectrum are presented .
	manualset3
196945	4	416112	7	NULL	NULL	0	NULL	band origins	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Updated tables of vibrational energy levels , molecular constants , band origins , and intensities for carbon dioxide in the infrared region of the spectrum are presented .
	manualset3
196946	5	416112	7	NULL	NULL	0	NULL	intensities	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Updated tables of vibrational energy levels , molecular constants , band origins , and intensities for carbon dioxide in the infrared region of the spectrum are presented .
	manualset3
196947	6	416112	7	NULL	NULL	0	NULL	carbon dioxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Updated tables of vibrational energy levels , molecular constants , band origins , and intensities for carbon dioxide in the infrared region of the spectrum are presented .
	manualset3
196948	7	416112	7	NULL	NULL	0	NULL	infrared region 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Updated tables of vibrational energy levels , molecular constants , band origins , and intensities for carbon dioxide in the infrared region of the spectrum are presented .
	manualset3
196949	8	416112	7	NULL	NULL	0	NULL	spectrum	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Updated tables of vibrational energy levels , molecular constants , band origins , and intensities for carbon dioxide in the infrared region of the spectrum are presented .
	manualset3
196950	1	416113	7	NULL	NULL	0	NULL	Upgrade	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Upgrade of the extraction system of permanent magnet electron cyclotron resonance ion source .
	manualset3
196951	2	416113	7	NULL	NULL	NULL	NULL	extraction system	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Upgrade of the extraction system of permanent magnet electron cyclotron resonance ion source .
	manualset3
196952	3	416113	7	NULL	NULL	NULL	NULL	permanent magnet electron cyclotron resonance ion source	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Upgrade of the extraction system of permanent magnet electron cyclotron resonance ion source .
	manualset3
196953	1	416114	7	NULL	NULL	0	NULL	FCS addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon FCS addition , c-myc mRNAs slightly increased in the first 30 minutes , peaked at 75 minutes ( 2.2 fold induction ) and returned to the control value within 24 hours .
	manualset3
196954	2	416114	7	NULL	NULL	0	NULL	c-myc mRNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon FCS addition , c-myc mRNAs slightly increased in the first 30 minutes , peaked at 75 minutes ( 2.2 fold induction ) and returned to the control value within 24 hours .
	manualset3
196955	3	416114	7	NULL	NULL	0	NULL	 first 30 minutes	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon FCS addition , c-myc mRNAs slightly increased in the first 30 minutes , peaked at 75 minutes ( 2.2 fold induction ) and returned to the control value within 24 hours .
	manualset3
196956	4	416114	7	NULL	NULL	0	NULL	 75 minutes	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon FCS addition , c-myc mRNAs slightly increased in the first 30 minutes , peaked at 75 minutes ( 2.2 fold induction ) and returned to the control value within 24 hours .
	manualset3
196957	5	416114	7	NULL	NULL	0	NULL	2.2 fold induction	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon FCS addition , c-myc mRNAs slightly increased in the first 30 minutes , peaked at 75 minutes ( 2.2 fold induction ) and returned to the control value within 24 hours .
	manualset3
196958	6	416114	7	NULL	NULL	0	NULL	control value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon FCS addition , c-myc mRNAs slightly increased in the first 30 minutes , peaked at 75 minutes ( 2.2 fold induction ) and returned to the control value within 24 hours .
	manualset3
196959	7	416114	7	NULL	NULL	0	NULL	24 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon FCS addition , c-myc mRNAs slightly increased in the first 30 minutes , peaked at 75 minutes ( 2.2 fold induction ) and returned to the control value within 24 hours .
	manualset3
196960	1	416115	7	NULL	NULL	0	NULL	UVR exposure	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon UVR exposure , significant melanin production was measured within one hour ; cellular melanin continued to increase in a retinal - and calcium-dependent manner up to 5-fold after 24hr .
	manualset3
196961	2	416115	7	NULL	NULL	0	NULL	melanin production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon UVR exposure , significant melanin production was measured within one hour ; cellular melanin continued to increase in a retinal - and calcium-dependent manner up to 5-fold after 24hr .
	manualset3
196962	3	416115	7	NULL	NULL	0	NULL	one hour	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon UVR exposure , significant melanin production was measured within one hour ; cellular melanin continued to increase in a retinal - and calcium-dependent manner up to 5-fold after 24hr .
	manualset3
196963	4	416115	7	NULL	NULL	0	NULL	 cellular melanin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon UVR exposure , significant melanin production was measured within one hour ; cellular melanin continued to increase in a retinal - and calcium-dependent manner up to 5-fold after 24hr .
	manualset3
196964	5	416115	7	NULL	NULL	0	NULL	retinal -dependent manner	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon UVR exposure , significant melanin production was measured within one hour ; cellular melanin continued to increase in a retinal - and calcium-dependent manner up to 5-fold after 24hr .
	manualset3
196965	6	416115	7	NULL	NULL	0	NULL	calcium-dependent manner	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon UVR exposure , significant melanin production was measured within one hour ; cellular melanin continued to increase in a retinal - and calcium-dependent manner up to 5-fold after 24hr .
	manualset3
196966	7	416115	7	NULL	NULL	0	NULL	5-fold 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon UVR exposure , significant melanin production was measured within one hour ; cellular melanin continued to increase in a retinal - and calcium-dependent manner up to 5-fold after 24hr .
	manualset3
196967	8	416115	7	NULL	NULL	0	NULL	24hr 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon UVR exposure , significant melanin production was measured within one hour ; cellular melanin continued to increase in a retinal - and calcium-dependent manner up to 5-fold after 24hr .
	manualset3
196968	1	416116	7	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon binding , nuclear receptors modulate transcription through affecting the local chromatin environment via recruitment of various coregulatory proteins .
	manualset3
196969	2	416116	7	NULL	NULL	0	NULL	nuclear receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon binding , nuclear receptors modulate transcription through affecting the local chromatin environment via recruitment of various coregulatory proteins .
	manualset3
196970	3	416116	7	NULL	NULL	0	NULL	transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon binding , nuclear receptors modulate transcription through affecting the local chromatin environment via recruitment of various coregulatory proteins .
	manualset3
196971	4	416116	7	NULL	NULL	0	NULL	local chromatin environment 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon binding , nuclear receptors modulate transcription through affecting the local chromatin environment via recruitment of various coregulatory proteins .
	manualset3
196972	5	416116	7	NULL	NULL	0	NULL	 recruitment	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon binding , nuclear receptors modulate transcription through affecting the local chromatin environment via recruitment of various coregulatory proteins .
	manualset3
196973	6	416116	7	NULL	NULL	0	NULL	coregulatory proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon binding , nuclear receptors modulate transcription through affecting the local chromatin environment via recruitment of various coregulatory proteins .
	manualset3
196974	1	416117	7	NULL	NULL	0	NULL	detection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon detection of a mass , distinguishing the cyst from the solid mass ( often by fine-needle aspiration or FNAB ) is one of the most important tasks facing the clinician .
	manualset3
196975	2	416117	7	NULL	NULL	0	NULL	mass 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon detection of a mass , distinguishing the cyst from the solid mass ( often by fine-needle aspiration or FNAB ) is one of the most important tasks facing the clinician .
	manualset3
196976	3	416117	7	NULL	NULL	0	NULL	cyst	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon detection of a mass , distinguishing the cyst from the solid mass ( often by fine-needle aspiration or FNAB ) is one of the most important tasks facing the clinician .
	manualset3
196977	4	416117	7	NULL	NULL	0	NULL	solid mass	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon detection of a mass , distinguishing the cyst from the solid mass ( often by fine-needle aspiration or FNAB ) is one of the most important tasks facing the clinician .
	manualset3
196978	5	416117	7	NULL	NULL	0	NULL	fine-needle aspiration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon detection of a mass , distinguishing the cyst from the solid mass ( often by fine-needle aspiration or FNAB ) is one of the most important tasks facing the clinician .
	manualset3
196979	6	416117	7	NULL	NULL	0	NULL	FNAB	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon detection of a mass , distinguishing the cyst from the solid mass ( often by fine-needle aspiration or FNAB ) is one of the most important tasks facing the clinician .
	manualset3
196980	7	416117	7	NULL	NULL	0	NULL	tasks	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon detection of a mass , distinguishing the cyst from the solid mass ( often by fine-needle aspiration or FNAB ) is one of the most important tasks facing the clinician .
	manualset3
196981	8	416117	7	NULL	NULL	0	NULL	clinician	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon detection of a mass , distinguishing the cyst from the solid mass ( often by fine-needle aspiration or FNAB ) is one of the most important tasks facing the clinician .
	manualset3
196982	9	416117	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon detection of a mass , distinguishing the cyst from the solid mass ( often by fine-needle aspiration or FNAB ) is one of the most important tasks facing the clinician .
	manualset3
196983	1	416118	7	NULL	NULL	0	NULL	inclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon inclusion of scalar relativistic effects ( -3 cm ( -1 ) on omega ( e ) ) , a potential curve of spectroscopic quality ( sub-cm ( -1 ) accuracy ) is obtained .
	manualset3
196984	2	416118	7	NULL	NULL	0	NULL	scalar relativistic effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon inclusion of scalar relativistic effects ( -3 cm ( -1 ) on omega ( e ) ) , a potential curve of spectroscopic quality ( sub-cm ( -1 ) accuracy ) is obtained .
	manualset3
196985	3	416118	7	NULL	NULL	0	NULL	 -3 cm ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon inclusion of scalar relativistic effects ( -3 cm ( -1 ) on omega ( e ) ) , a potential curve of spectroscopic quality ( sub-cm ( -1 ) accuracy ) is obtained .
	manualset3
196986	4	416118	7	NULL	NULL	NULL	NULL	omega ( e ) 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Upon inclusion of scalar relativistic effects ( -3 cm ( -1 ) on omega ( e ) ) , a potential curve of spectroscopic quality ( sub-cm ( -1 ) accuracy ) is obtained .
	manualset3
196987	5	416118	7	NULL	NULL	0	NULL	potential curve	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon inclusion of scalar relativistic effects ( -3 cm ( -1 ) on omega ( e ) ) , a potential curve of spectroscopic quality ( sub-cm ( -1 ) accuracy ) is obtained .
	manualset3
196988	6	416118	7	NULL	NULL	0	NULL	spectroscopic quality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon inclusion of scalar relativistic effects ( -3 cm ( -1 ) on omega ( e ) ) , a potential curve of spectroscopic quality ( sub-cm ( -1 ) accuracy ) is obtained .
	manualset3
196989	7	416118	7	NULL	NULL	0	NULL	sub-cm ( -1 ) accuracy 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon inclusion of scalar relativistic effects ( -3 cm ( -1 ) on omega ( e ) ) , a potential curve of spectroscopic quality ( sub-cm ( -1 ) accuracy ) is obtained .
	manualset3
196990	1	416119	7	NULL	NULL	0	NULL	removal 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon removal of the organic solvent , stable and homogenously sized ( 70-100 nm ) lipid-nucleic acid nanoparticles ( Genospheres ) were formed .
	manualset3
196991	2	416119	7	NULL	NULL	0	NULL	organic solvent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon removal of the organic solvent , stable and homogenously sized ( 70-100 nm ) lipid-nucleic acid nanoparticles ( Genospheres ) were formed .
	manualset3
196992	3	416119	7	NULL	NULL	NULL	NULL	stable and homogenously sized 70-100 nm	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Upon removal of the organic solvent , stable and homogenously sized ( 70-100 nm ) lipid-nucleic acid nanoparticles ( Genospheres ) were formed .
	manualset3
196993	4	416119	7	NULL	NULL	0	NULL	 lipid-nucleic acid nanoparticles	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon removal of the organic solvent , stable and homogenously sized ( 70-100 nm ) lipid-nucleic acid nanoparticles ( Genospheres ) were formed .
	manualset3
196994	5	416119	7	NULL	NULL	0	NULL	Genospheres	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon removal of the organic solvent , stable and homogenously sized ( 70-100 nm ) lipid-nucleic acid nanoparticles ( Genospheres ) were formed .
	manualset3
196995	1	416120	7	NULL	NULL	0	NULL	 procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After the procedure , pain relief was reported in 25 ( 93 % ) patients .
	manualset3
196996	2	416120	7	NULL	NULL	0	NULL	pain relief	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After the procedure , pain relief was reported in 25 ( 93 % ) patients .
	manualset3
196997	3	416120	7	NULL	NULL	0	NULL	25 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	After the procedure , pain relief was reported in 25 ( 93 % ) patients .
	manualset3
196998	4	416120	7	NULL	NULL	0	NULL	93 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After the procedure , pain relief was reported in 25 ( 93 % ) patients .
	manualset3
196999	1	416121	7	NULL	NULL	0	NULL	soil drying	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon soil drying , plants can reduce water consumption by minimizing transpiration through stomata , the closable pores of the leaf .
	manualset3
197000	2	416121	7	NULL	NULL	0	NULL	plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon soil drying , plants can reduce water consumption by minimizing transpiration through stomata , the closable pores of the leaf .
	manualset3
197001	3	416121	7	NULL	NULL	0	NULL	 water consumption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon soil drying , plants can reduce water consumption by minimizing transpiration through stomata , the closable pores of the leaf .
	manualset3
197002	4	416121	7	NULL	NULL	0	NULL	transpiration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon soil drying , plants can reduce water consumption by minimizing transpiration through stomata , the closable pores of the leaf .
	manualset3
197003	5	416121	7	NULL	NULL	0	NULL	stomata	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon soil drying , plants can reduce water consumption by minimizing transpiration through stomata , the closable pores of the leaf .
	manualset3
197004	6	416121	7	NULL	NULL	0	NULL	closable pores	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon soil drying , plants can reduce water consumption by minimizing transpiration through stomata , the closable pores of the leaf .
	manualset3
197005	7	416121	7	NULL	NULL	0	NULL	leaf	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon soil drying , plants can reduce water consumption by minimizing transpiration through stomata , the closable pores of the leaf .
	manualset3
197058	1	416122	7	NULL	NULL	0	NULL	stimulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon stimulation of the medial giant nerve fiber , NAAG is the primary radioactive metabolite released .
	manualset3
197059	2	416122	7	NULL	NULL	0	NULL	medial giant nerve fiber	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon stimulation of the medial giant nerve fiber , NAAG is the primary radioactive metabolite released .
	manualset3
197060	3	416122	7	NULL	NULL	0	NULL	NAAG	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon stimulation of the medial giant nerve fiber , NAAG is the primary radioactive metabolite released .
	manualset3
197061	4	416122	7	NULL	NULL	0	NULL	primary radioactive metabolite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon stimulation of the medial giant nerve fiber , NAAG is the primary radioactive metabolite released .
	manualset3
197062	1	416123	7	NULL	NULL	0	NULL	Upregulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Upregulation of the GFAP was not noticed until 2 days after compression .
	manualset3
197063	2	416123	7	NULL	NULL	0	NULL	GFAP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Upregulation of the GFAP was not noticed until 2 days after compression .
	manualset3
197064	3	416123	7	NULL	NULL	0	NULL	2 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Upregulation of the GFAP was not noticed until 2 days after compression .
	manualset3
197065	4	416123	7	NULL	NULL	0	NULL	 compression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Upregulation of the GFAP was not noticed until 2 days after compression .
	manualset3
197066	1	416124	7	NULL	NULL	0	NULL	Upregulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Upregulation of the heme oxygenase system ameliorates postprandial and fasting hyperglycemia in type 2 diabetes .
	manualset3
197067	2	416124	7	NULL	NULL	0	NULL	heme oxygenase system	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Upregulation of the heme oxygenase system ameliorates postprandial and fasting hyperglycemia in type 2 diabetes .
	manualset3
197068	3	416124	7	NULL	NULL	0	NULL	postprandial hyperglycemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Upregulation of the heme oxygenase system ameliorates postprandial and fasting hyperglycemia in type 2 diabetes .
	manualset3
197069	4	416124	7	NULL	NULL	0	NULL	fasting hyperglycemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Upregulation of the heme oxygenase system ameliorates postprandial and fasting hyperglycemia in type 2 diabetes .
	manualset3
197070	5	416124	7	NULL	NULL	0	NULL	 type 2 diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Upregulation of the heme oxygenase system ameliorates postprandial and fasting hyperglycemia in type 2 diabetes .
	manualset3
197071	1	416125	7	NULL	NULL	0	NULL	Upstream binding factor	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Upstream binding factor up-regulated in hepatocellular carcinoma is related to the survival and cisplatin-sensitivity of cancer cells .
	manualset3
197072	2	416125	7	NULL	NULL	0	NULL	hepatocellular carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Upstream binding factor up-regulated in hepatocellular carcinoma is related to the survival and cisplatin-sensitivity of cancer cells .
	manualset3
197073	3	416125	7	NULL	NULL	0	NULL	survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Upstream binding factor up-regulated in hepatocellular carcinoma is related to the survival and cisplatin-sensitivity of cancer cells .
	manualset3
197074	4	416125	7	NULL	NULL	0	NULL	cisplatin-sensitivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Upstream binding factor up-regulated in hepatocellular carcinoma is related to the survival and cisplatin-sensitivity of cancer cells .
	manualset3
197075	5	416125	7	NULL	NULL	0	NULL	cancer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Upstream binding factor up-regulated in hepatocellular carcinoma is related to the survival and cisplatin-sensitivity of cancer cells .
	manualset3
197076	1	416126	7	NULL	NULL	0	NULL	Uptake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Uptake and efflux of ( ( 3 ) H ) methionine and ( ( 14 ) C ) MeHg-L-cysteine were trans - stimulated by leucine and phenylalanine , but not by glutamate , indicating that MeHg-L-cysteine is both a cis - and trans - substrate .
	manualset3
197077	2	416126	7	NULL	NULL	0	NULL	efflux	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Uptake and efflux of ( ( 3 ) H ) methionine and ( ( 14 ) C ) MeHg-L-cysteine were trans - stimulated by leucine and phenylalanine , but not by glutamate , indicating that MeHg-L-cysteine is both a cis - and trans - substrate .
	manualset3
197078	3	416126	7	NULL	NULL	0	NULL	 ( ( 3 ) H ) methionine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Uptake and efflux of ( ( 3 ) H ) methionine and ( ( 14 ) C ) MeHg-L-cysteine were trans - stimulated by leucine and phenylalanine , but not by glutamate , indicating that MeHg-L-cysteine is both a cis - and trans - substrate .
	manualset3
197079	4	416126	7	NULL	NULL	NULL	NULL	 ( ( 14 ) C ) MeHg-L-cysteine	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Uptake and efflux of ( ( 3 ) H ) methionine and ( ( 14 ) C ) MeHg-L-cysteine were trans - stimulated by leucine and phenylalanine , but not by glutamate , indicating that MeHg-L-cysteine is both a cis - and trans - substrate .
	manualset3
197080	5	416126	7	NULL	NULL	0	NULL	leucine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Uptake and efflux of ( ( 3 ) H ) methionine and ( ( 14 ) C ) MeHg-L-cysteine were trans - stimulated by leucine and phenylalanine , but not by glutamate , indicating that MeHg-L-cysteine is both a cis - and trans - substrate .
	manualset3
197081	6	416126	7	NULL	NULL	0	NULL	phenylalanine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Uptake and efflux of ( ( 3 ) H ) methionine and ( ( 14 ) C ) MeHg-L-cysteine were trans - stimulated by leucine and phenylalanine , but not by glutamate , indicating that MeHg-L-cysteine is both a cis - and trans - substrate .
	manualset3
197082	7	416126	7	NULL	NULL	0	NULL	glutamate	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Uptake and efflux of ( ( 3 ) H ) methionine and ( ( 14 ) C ) MeHg-L-cysteine were trans - stimulated by leucine and phenylalanine , but not by glutamate , indicating that MeHg-L-cysteine is both a cis - and trans - substrate .
	manualset3
197083	8	416126	7	NULL	NULL	0	NULL	MeHg-L-cysteine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Uptake and efflux of ( ( 3 ) H ) methionine and ( ( 14 ) C ) MeHg-L-cysteine were trans - stimulated by leucine and phenylalanine , but not by glutamate , indicating that MeHg-L-cysteine is both a cis - and trans - substrate .
	manualset3
197084	9	416126	7	NULL	NULL	NULL	NULL	 cis - substrate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Uptake and efflux of ( ( 3 ) H ) methionine and ( ( 14 ) C ) MeHg-L-cysteine were trans - stimulated by leucine and phenylalanine , but not by glutamate , indicating that MeHg-L-cysteine is both a cis - and trans - substrate .
	manualset3
197085	10	416126	7	NULL	NULL	NULL	NULL	trans - substrate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Uptake and efflux of ( ( 3 ) H ) methionine and ( ( 14 ) C ) MeHg-L-cysteine were trans - stimulated by leucine and phenylalanine , but not by glutamate , indicating that MeHg-L-cysteine is both a cis - and trans - substrate .
	manualset3
197086	1	416127	7	NULL	NULL	0	NULL	Uptake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Uptake and metabolism of retinol in cultured Sertoli cells : evidence for a kinetic model .
	manualset3
197087	2	416127	7	NULL	NULL	0	NULL	metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Uptake and metabolism of retinol in cultured Sertoli cells : evidence for a kinetic model .
	manualset3
197088	3	416127	7	NULL	NULL	0	NULL	retinol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Uptake and metabolism of retinol in cultured Sertoli cells : evidence for a kinetic model .
	manualset3
197089	4	416127	7	NULL	NULL	0	NULL	cultured Sertoli cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Uptake and metabolism of retinol in cultured Sertoli cells : evidence for a kinetic model .
	manualset3
197090	5	416127	7	NULL	NULL	0	NULL	evidence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Uptake and metabolism of retinol in cultured Sertoli cells : evidence for a kinetic model .
	manualset3
197091	6	416127	7	NULL	NULL	0	NULL	kinetic model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Uptake and metabolism of retinol in cultured Sertoli cells : evidence for a kinetic model .
	manualset3
197092	1	416128	7	NULL	NULL	0	NULL	Uptake 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Uptake of the negatively charged amino acid L-glutamate , the neutral amino acid L-serine , and the positively charged amino acid L-arginine was examined in membrane vesicles fused with cytochrome c-containing liposomes .
	manualset3
197093	2	416128	7	NULL	NULL	0	NULL	 negatively charged amino acid L-glutamate	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Uptake of the negatively charged amino acid L-glutamate , the neutral amino acid L-serine , and the positively charged amino acid L-arginine was examined in membrane vesicles fused with cytochrome c-containing liposomes .
	manualset3
197094	3	416128	7	NULL	NULL	0	NULL	neutral amino acid L-serine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Uptake of the negatively charged amino acid L-glutamate , the neutral amino acid L-serine , and the positively charged amino acid L-arginine was examined in membrane vesicles fused with cytochrome c-containing liposomes .
	manualset3
197095	4	416128	7	NULL	NULL	0	NULL	positively charged amino acid L-arginine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Uptake of the negatively charged amino acid L-glutamate , the neutral amino acid L-serine , and the positively charged amino acid L-arginine was examined in membrane vesicles fused with cytochrome c-containing liposomes .
	manualset3
197096	5	416128	7	NULL	NULL	0	NULL	membrane vesicles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Uptake of the negatively charged amino acid L-glutamate , the neutral amino acid L-serine , and the positively charged amino acid L-arginine was examined in membrane vesicles fused with cytochrome c-containing liposomes .
	manualset3
197097	6	416128	7	NULL	NULL	0	NULL	cytochrome c-containing liposomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Uptake of the negatively charged amino acid L-glutamate , the neutral amino acid L-serine , and the positively charged amino acid L-arginine was examined in membrane vesicles fused with cytochrome c-containing liposomes .
	manualset3
197133	2	416129	7	NULL	NULL	NULL	NULL	sleep patterns	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After the rapid 9-h phase advance , sleep patterns , temperature amplitude , aMT6s acrophase , alertness , and performance took at least 5 days to reestablish normal baseline patterns .
	manualset3
197135	1	416129	7	NULL	NULL	NULL	NULL	 rapid 9-h phase advance	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After the rapid 9-h phase advance , sleep patterns , temperature amplitude , aMT6s acrophase , alertness , and performance took at least 5 days to reestablish normal baseline patterns .
	manualset3
197139	3	416129	7	NULL	NULL	0	NULL	 temperature amplitude 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After the rapid 9-h phase advance , sleep patterns , temperature amplitude , aMT6s acrophase , alertness , and performance took at least 5 days to reestablish normal baseline patterns .
	manualset3
197142	4	416129	7	NULL	NULL	0	NULL	aMT6s acrophase	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After the rapid 9-h phase advance , sleep patterns , temperature amplitude , aMT6s acrophase , alertness , and performance took at least 5 days to reestablish normal baseline patterns .
	manualset3
197143	5	416129	7	NULL	NULL	0	NULL	alertness	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After the rapid 9-h phase advance , sleep patterns , temperature amplitude , aMT6s acrophase , alertness , and performance took at least 5 days to reestablish normal baseline patterns .
	manualset3
197145	6	416129	7	NULL	NULL	0	NULL	 performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After the rapid 9-h phase advance , sleep patterns , temperature amplitude , aMT6s acrophase , alertness , and performance took at least 5 days to reestablish normal baseline patterns .
	manualset3
197148	7	416129	7	NULL	NULL	0	NULL	5 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After the rapid 9-h phase advance , sleep patterns , temperature amplitude , aMT6s acrophase , alertness , and performance took at least 5 days to reestablish normal baseline patterns .
	manualset3
197150	8	416129	7	NULL	NULL	0	NULL	normal baseline patterns	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After the rapid 9-h phase advance , sleep patterns , temperature amplitude , aMT6s acrophase , alertness , and performance took at least 5 days to reestablish normal baseline patterns .
	manualset3
197158	1	416130	7	NULL	NULL	0	NULL	Urban adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Urban adults have a higher probability of being overweight ( OR = 1.18 , P & lt ; .01 ) and having hypertension ( OR = 1.19 , P & lt ; .1 ) .
	manualset3
197159	2	416130	7	NULL	NULL	0	NULL	higher probability	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Urban adults have a higher probability of being overweight ( OR = 1.18 , P & lt ; .01 ) and having hypertension ( OR = 1.19 , P & lt ; .1 ) .
	manualset3
197160	3	416130	7	NULL	NULL	0	NULL	overweight	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Urban adults have a higher probability of being overweight ( OR = 1.18 , P & lt ; .01 ) and having hypertension ( OR = 1.19 , P & lt ; .1 ) .
	manualset3
197161	4	416130	7	NULL	NULL	0	NULL	 OR = 1.18 , P & lt ; .01	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Urban adults have a higher probability of being overweight ( OR = 1.18 , P & lt ; .01 ) and having hypertension ( OR = 1.19 , P & lt ; .1 ) .
	manualset3
197162	5	416130	7	NULL	NULL	0	NULL	hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Urban adults have a higher probability of being overweight ( OR = 1.18 , P & lt ; .01 ) and having hypertension ( OR = 1.19 , P & lt ; .1 ) .
	manualset3
197163	6	416130	7	NULL	NULL	0	NULL	OR = 1.19 , P & lt ; .1	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Urban adults have a higher probability of being overweight ( OR = 1.18 , P & lt ; .01 ) and having hypertension ( OR = 1.19 , P & lt ; .1 ) .
	manualset3
197261	1	416131	7	NULL	NULL	0	NULL	Urea-type ligand-modified CdSe quantum dots	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Urea-type ligand-modified CdSe quantum dots as a fluorescence `` turn-on '' sensor for CO3 ( 2 - ) anions .
	manualset3
197262	2	416131	7	NULL	NULL	0	NULL	fluorescence `	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Urea-type ligand-modified CdSe quantum dots as a fluorescence `` turn-on '' sensor for CO3 ( 2 - ) anions .
	manualset3
197263	3	416131	7	NULL	NULL	0	NULL	 `` turn-on '' sensor	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Urea-type ligand-modified CdSe quantum dots as a fluorescence `` turn-on '' sensor for CO3 ( 2 - ) anions .
	manualset3
197264	4	416131	7	NULL	NULL	0	NULL	CO3 ( 2 - ) anions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Urea-type ligand-modified CdSe quantum dots as a fluorescence `` turn-on '' sensor for CO3 ( 2 - ) anions .
	manualset3
197265	1	416132	7	NULL	NULL	0	NULL	Urinary alpha1-antichymotrypsin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary alpha1-antichymotrypsin : a biomarker of prion infection .
	manualset3
197266	2	416132	7	NULL	NULL	0	NULL	biomarker	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary alpha1-antichymotrypsin : a biomarker of prion infection .
	manualset3
197267	3	416132	7	NULL	NULL	0	NULL	prion infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary alpha1-antichymotrypsin : a biomarker of prion infection .
	manualset3
197268	1	416133	7	NULL	NULL	0	NULL	Urinary cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary cultures , urinalysis , three-glass test , and investigation of the prostate secretion , Mycobacteria culture , and susceptibility testing were performed in all 514 patients .
	manualset3
197269	2	416133	7	NULL	NULL	0	NULL	urinalysis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary cultures , urinalysis , three-glass test , and investigation of the prostate secretion , Mycobacteria culture , and susceptibility testing were performed in all 514 patients .
	manualset3
197270	3	416133	7	NULL	NULL	0	NULL	three-glass test	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary cultures , urinalysis , three-glass test , and investigation of the prostate secretion , Mycobacteria culture , and susceptibility testing were performed in all 514 patients .
	manualset3
197271	4	416133	7	NULL	NULL	0	NULL	investigation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary cultures , urinalysis , three-glass test , and investigation of the prostate secretion , Mycobacteria culture , and susceptibility testing were performed in all 514 patients .
	manualset3
197272	5	416133	7	NULL	NULL	0	NULL	prostate secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary cultures , urinalysis , three-glass test , and investigation of the prostate secretion , Mycobacteria culture , and susceptibility testing were performed in all 514 patients .
	manualset3
197273	6	416133	7	NULL	NULL	0	NULL	Mycobacteria culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary cultures , urinalysis , three-glass test , and investigation of the prostate secretion , Mycobacteria culture , and susceptibility testing were performed in all 514 patients .
	manualset3
197274	7	416133	7	NULL	NULL	0	NULL	susceptibility testing 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary cultures , urinalysis , three-glass test , and investigation of the prostate secretion , Mycobacteria culture , and susceptibility testing were performed in all 514 patients .
	manualset3
197275	8	416133	7	NULL	NULL	0	NULL	514 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary cultures , urinalysis , three-glass test , and investigation of the prostate secretion , Mycobacteria culture , and susceptibility testing were performed in all 514 patients .
	manualset3
197276	1	416134	7	NULL	NULL	0	NULL	Urinary excretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary excretion of nitrogen , urea , creatinine and 3-MH were not affected by the histidine-free diet .
	manualset3
197277	2	416134	7	NULL	NULL	0	NULL	 nitrogen	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary excretion of nitrogen , urea , creatinine and 3-MH were not affected by the histidine-free diet .
	manualset3
197278	3	416134	7	NULL	NULL	0	NULL	 urea	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary excretion of nitrogen , urea , creatinine and 3-MH were not affected by the histidine-free diet .
	manualset3
197279	4	416134	7	NULL	NULL	0	NULL	creatinine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary excretion of nitrogen , urea , creatinine and 3-MH were not affected by the histidine-free diet .
	manualset3
197280	5	416134	7	NULL	NULL	0	NULL	3-MH	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary excretion of nitrogen , urea , creatinine and 3-MH were not affected by the histidine-free diet .
	manualset3
197281	6	416134	7	NULL	NULL	0	NULL	histidine-free diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary excretion of nitrogen , urea , creatinine and 3-MH were not affected by the histidine-free diet .
	manualset3
197282	1	416135	7	NULL	NULL	0	NULL	stabilization period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After the stabilization period the men were split into two groups , one group continued on the stabilization diet while the other received the salmon diet that contained approximately 2.1 energy percent ( En % ) of calories from 20 - and 22-carbon n-3 fatty acids .
	manualset3
197283	2	416135	7	NULL	NULL	0	NULL	 men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	After the stabilization period the men were split into two groups , one group continued on the stabilization diet while the other received the salmon diet that contained approximately 2.1 energy percent ( En % ) of calories from 20 - and 22-carbon n-3 fatty acids .
	manualset3
197284	3	416135	7	NULL	NULL	0	NULL	 two groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	After the stabilization period the men were split into two groups , one group continued on the stabilization diet while the other received the salmon diet that contained approximately 2.1 energy percent ( En % ) of calories from 20 - and 22-carbon n-3 fatty acids .
	manualset3
197285	4	416135	7	NULL	NULL	0	NULL	one group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	After the stabilization period the men were split into two groups , one group continued on the stabilization diet while the other received the salmon diet that contained approximately 2.1 energy percent ( En % ) of calories from 20 - and 22-carbon n-3 fatty acids .
	manualset3
197286	5	416135	7	NULL	NULL	0	NULL	stabilization diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	After the stabilization period the men were split into two groups , one group continued on the stabilization diet while the other received the salmon diet that contained approximately 2.1 energy percent ( En % ) of calories from 20 - and 22-carbon n-3 fatty acids .
	manualset3
197287	6	416135	7	NULL	NULL	0	NULL	salmon diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	After the stabilization period the men were split into two groups , one group continued on the stabilization diet while the other received the salmon diet that contained approximately 2.1 energy percent ( En % ) of calories from 20 - and 22-carbon n-3 fatty acids .
	manualset3
197288	7	416135	7	NULL	NULL	0	NULL	2.1 energy percent ( En % ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After the stabilization period the men were split into two groups , one group continued on the stabilization diet while the other received the salmon diet that contained approximately 2.1 energy percent ( En % ) of calories from 20 - and 22-carbon n-3 fatty acids .
	manualset3
197289	8	416135	7	NULL	NULL	0	NULL	calories	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After the stabilization period the men were split into two groups , one group continued on the stabilization diet while the other received the salmon diet that contained approximately 2.1 energy percent ( En % ) of calories from 20 - and 22-carbon n-3 fatty acids .
	manualset3
197290	9	416135	7	NULL	NULL	NULL	NULL	20 -carbon n-3 fatty acids	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After the stabilization period the men were split into two groups , one group continued on the stabilization diet while the other received the salmon diet that contained approximately 2.1 energy percent ( En % ) of calories from 20 - and 22-carbon n-3 fatty acids .
	manualset3
200230	10	416135	7	NULL	NULL	0	NULL	22-carbon n-3 fatty acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After the stabilization period the men were split into two groups , one group continued on the stabilization diet while the other received the salmon diet that contained approximately 2.1 energy percent ( En % ) of calories from 20 - and 22-carbon n-3 fatty acids .
	manualset3
197291	1	416136	7	NULL	NULL	NULL	NULL	Urinary measurements	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Urinary measurements of HVA , vanillylmandelic acid , and catecholamines can lead to false-negative conclusions .
	manualset3
197292	2	416136	7	NULL	NULL	0	NULL	HVA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary measurements of HVA , vanillylmandelic acid , and catecholamines can lead to false-negative conclusions .
	manualset3
197293	3	416136	7	NULL	NULL	0	NULL	vanillylmandelic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary measurements of HVA , vanillylmandelic acid , and catecholamines can lead to false-negative conclusions .
	manualset3
197294	4	416136	7	NULL	NULL	0	NULL	catecholamines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary measurements of HVA , vanillylmandelic acid , and catecholamines can lead to false-negative conclusions .
	manualset3
197295	5	416136	7	NULL	NULL	0	NULL	false-negative conclusions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary measurements of HVA , vanillylmandelic acid , and catecholamines can lead to false-negative conclusions .
	manualset3
197296	1	416137	7	NULL	NULL	0	NULL	Urinary methylmalonic acid ( MMA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary methylmalonic acid ( MMA ) and 4-hydroxyphenyllactic acid ( HPL ) have been determined in 3345 and 2498 3-week-old newborns , respectively .
	manualset3
197297	2	416137	7	NULL	NULL	0	NULL	4-hydroxyphenyllactic acid ( HPL )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary methylmalonic acid ( MMA ) and 4-hydroxyphenyllactic acid ( HPL ) have been determined in 3345 and 2498 3-week-old newborns , respectively .
	manualset3
197298	3	416137	7	NULL	NULL	0	NULL	3345	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary methylmalonic acid ( MMA ) and 4-hydroxyphenyllactic acid ( HPL ) have been determined in 3345 and 2498 3-week-old newborns , respectively .
	manualset3
197299	4	416137	7	NULL	NULL	0	NULL	2498	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary methylmalonic acid ( MMA ) and 4-hydroxyphenyllactic acid ( HPL ) have been determined in 3345 and 2498 3-week-old newborns , respectively .
	manualset3
197300	5	416137	7	NULL	NULL	0	NULL	3-week-old newborns	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary methylmalonic acid ( MMA ) and 4-hydroxyphenyllactic acid ( HPL ) have been determined in 3345 and 2498 3-week-old newborns , respectively .
	manualset3
197301	1	416138	7	NULL	NULL	0	NULL	Urinary oxalate concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary oxalate concentrations were significantly ( P less than 0.05 ) higher in patients with Crohn 's disease and steatorrhoea , but not in those with chronic pancreatitis , after administrating a high-oxalate diet compared with healthy subjects .
	manualset3
197302	2	416138	7	NULL	NULL	0	NULL	P less than 0.05	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary oxalate concentrations were significantly ( P less than 0.05 ) higher in patients with Crohn 's disease and steatorrhoea , but not in those with chronic pancreatitis , after administrating a high-oxalate diet compared with healthy subjects .
	manualset3
197303	3	416138	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary oxalate concentrations were significantly ( P less than 0.05 ) higher in patients with Crohn 's disease and steatorrhoea , but not in those with chronic pancreatitis , after administrating a high-oxalate diet compared with healthy subjects .
	manualset3
197304	4	416138	7	NULL	NULL	0	NULL	Crohn 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary oxalate concentrations were significantly ( P less than 0.05 ) higher in patients with Crohn 's disease and steatorrhoea , but not in those with chronic pancreatitis , after administrating a high-oxalate diet compared with healthy subjects .
	manualset3
197305	5	416138	7	NULL	NULL	0	NULL	steatorrhoea	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary oxalate concentrations were significantly ( P less than 0.05 ) higher in patients with Crohn 's disease and steatorrhoea , but not in those with chronic pancreatitis , after administrating a high-oxalate diet compared with healthy subjects .
	manualset3
197306	6	416138	7	NULL	NULL	0	NULL	chronic pancreatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary oxalate concentrations were significantly ( P less than 0.05 ) higher in patients with Crohn 's disease and steatorrhoea , but not in those with chronic pancreatitis , after administrating a high-oxalate diet compared with healthy subjects .
	manualset3
197307	7	416138	7	NULL	NULL	0	NULL	high-oxalate diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary oxalate concentrations were significantly ( P less than 0.05 ) higher in patients with Crohn 's disease and steatorrhoea , but not in those with chronic pancreatitis , after administrating a high-oxalate diet compared with healthy subjects .
	manualset3
197308	8	416138	7	NULL	NULL	0	NULL	healthy subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary oxalate concentrations were significantly ( P less than 0.05 ) higher in patients with Crohn 's disease and steatorrhoea , but not in those with chronic pancreatitis , after administrating a high-oxalate diet compared with healthy subjects .
	manualset3
197309	1	416139	7	NULL	NULL	0	NULL	Urinary tract infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary tract infections in women : diagnosis and management in primary care .
	manualset3
197310	2	416139	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary tract infections in women : diagnosis and management in primary care .
	manualset3
197311	3	416139	7	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary tract infections in women : diagnosis and management in primary care .
	manualset3
197312	4	416139	7	NULL	NULL	0	NULL	management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary tract infections in women : diagnosis and management in primary care .
	manualset3
197313	5	416139	7	NULL	NULL	0	NULL	primary care	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Urinary tract infections in women : diagnosis and management in primary care .
	manualset3
197314	1	416140	7	NULL	NULL	0	NULL	Urine samples	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Urine and serum samples from emergency room patients with neuropsychiatric symptoms and methadone clinic patients and autopsy material showed a significant incidence of PCP abuse , particularly among adolescents and young adults .
	manualset3
197315	2	416140	7	NULL	NULL	0	NULL	serum samples	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Urine and serum samples from emergency room patients with neuropsychiatric symptoms and methadone clinic patients and autopsy material showed a significant incidence of PCP abuse , particularly among adolescents and young adults .
	manualset3
197316	3	416140	7	NULL	NULL	0	NULL	emergency room patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Urine and serum samples from emergency room patients with neuropsychiatric symptoms and methadone clinic patients and autopsy material showed a significant incidence of PCP abuse , particularly among adolescents and young adults .
	manualset3
197317	4	416140	7	NULL	NULL	0	NULL	neuropsychiatric symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Urine and serum samples from emergency room patients with neuropsychiatric symptoms and methadone clinic patients and autopsy material showed a significant incidence of PCP abuse , particularly among adolescents and young adults .
	manualset3
197318	5	416140	7	NULL	NULL	0	NULL	methadone clinic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Urine and serum samples from emergency room patients with neuropsychiatric symptoms and methadone clinic patients and autopsy material showed a significant incidence of PCP abuse , particularly among adolescents and young adults .
	manualset3
197319	6	416140	7	NULL	NULL	0	NULL	autopsy material	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Urine and serum samples from emergency room patients with neuropsychiatric symptoms and methadone clinic patients and autopsy material showed a significant incidence of PCP abuse , particularly among adolescents and young adults .
	manualset3
197320	7	416140	7	NULL	NULL	0	NULL	significant incidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Urine and serum samples from emergency room patients with neuropsychiatric symptoms and methadone clinic patients and autopsy material showed a significant incidence of PCP abuse , particularly among adolescents and young adults .
	manualset3
197321	8	416140	7	NULL	NULL	0	NULL	 PCP abuse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Urine and serum samples from emergency room patients with neuropsychiatric symptoms and methadone clinic patients and autopsy material showed a significant incidence of PCP abuse , particularly among adolescents and young adults .
	manualset3
197322	9	416140	7	NULL	NULL	0	NULL	adolescents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Urine and serum samples from emergency room patients with neuropsychiatric symptoms and methadone clinic patients and autopsy material showed a significant incidence of PCP abuse , particularly among adolescents and young adults .
	manualset3
197323	10	416140	7	NULL	NULL	0	NULL	young adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Urine and serum samples from emergency room patients with neuropsychiatric symptoms and methadone clinic patients and autopsy material showed a significant incidence of PCP abuse , particularly among adolescents and young adults .
	manualset3
197324	1	416141	7	NULL	NULL	0	NULL	Urine concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Urine concentration of norfloxacin was determined periodically during serum acquisition periods .
	manualset3
197325	2	416141	7	NULL	NULL	0	NULL	norfloxacin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Urine concentration of norfloxacin was determined periodically during serum acquisition periods .
	manualset3
197326	3	416141	7	NULL	NULL	0	NULL	 serum acquisition periods	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Urine concentration of norfloxacin was determined periodically during serum acquisition periods .
	manualset3
197327	1	416142	7	NULL	NULL	0	NULL	Urine tryptophan color test	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Urine tryptophan color test in pregnancy and its clinical application .
	manualset3
197328	2	416142	7	NULL	NULL	0	NULL	 pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Urine tryptophan color test in pregnancy and its clinical application .
	manualset3
197329	3	416142	7	NULL	NULL	0	NULL	 clinical application	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Urine tryptophan color test in pregnancy and its clinical application .
	manualset3
197330	1	416143	7	NULL	NULL	NULL	NULL	Urocortin-1 ( UCN )	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Urocortin-1 ( UCN ) , a member of the corticotropin-releasing factor , is a cardioprotective peptide , and is also involved in cardiac hypertrophy .
	manualset3
197331	2	416143	7	NULL	NULL	NULL	NULL	member	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Urocortin-1 ( UCN ) , a member of the corticotropin-releasing factor , is a cardioprotective peptide , and is also involved in cardiac hypertrophy .
	manualset3
197332	3	416143	7	NULL	NULL	0	NULL	corticotropin-releasing factor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Urocortin-1 ( UCN ) , a member of the corticotropin-releasing factor , is a cardioprotective peptide , and is also involved in cardiac hypertrophy .
	manualset3
197333	4	416143	7	NULL	NULL	0	NULL	cardioprotective peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Urocortin-1 ( UCN ) , a member of the corticotropin-releasing factor , is a cardioprotective peptide , and is also involved in cardiac hypertrophy .
	manualset3
197334	5	416143	7	NULL	NULL	0	NULL	cardiac hypertrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Urocortin-1 ( UCN ) , a member of the corticotropin-releasing factor , is a cardioprotective peptide , and is also involved in cardiac hypertrophy .
	manualset3
197335	1	416144	7	NULL	NULL	0	NULL	Conservative surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Conservative surgery in ectopic pregnancy ) .
	manualset3
197336	2	416144	7	NULL	NULL	0	NULL	ectopic pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Conservative surgery in ectopic pregnancy ) .
	manualset3
197337	1	416145	7	NULL	NULL	0	NULL	switch  	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After the switch to tacrolimus , mean total cholesterol was reduced by 15 % at month 6 .
	manualset3
197338	2	416145	7	NULL	NULL	0	NULL	tacrolimus	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	After the switch to tacrolimus , mean total cholesterol was reduced by 15 % at month 6 .
	manualset3
197339	3	416145	7	NULL	NULL	0	NULL	mean total cholesterol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After the switch to tacrolimus , mean total cholesterol was reduced by 15 % at month 6 .
	manualset3
197340	4	416145	7	NULL	NULL	0	NULL	15 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After the switch to tacrolimus , mean total cholesterol was reduced by 15 % at month 6 .
	manualset3
197341	5	416145	7	NULL	NULL	0	NULL	month 6	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After the switch to tacrolimus , mean total cholesterol was reduced by 15 % at month 6 .
	manualset3
197342	1	416146	7	NULL	NULL	NULL	NULL	Urodynamic investigations	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Urodynamic investigations including cystometry and electronic simultaneous urethro-cystometry were made in 27 primiparae between 2 and 5 days after delivery to assess possible effects of lumbar epidural analgesia on the function of the lower urinary tract .
	manualset3
197343	2	416146	7	NULL	NULL	0	NULL	cystometry	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Urodynamic investigations including cystometry and electronic simultaneous urethro-cystometry were made in 27 primiparae between 2 and 5 days after delivery to assess possible effects of lumbar epidural analgesia on the function of the lower urinary tract .
	manualset3
197344	3	416146	7	NULL	NULL	0	NULL	electronic simultaneous urethro-cystometry	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Urodynamic investigations including cystometry and electronic simultaneous urethro-cystometry were made in 27 primiparae between 2 and 5 days after delivery to assess possible effects of lumbar epidural analgesia on the function of the lower urinary tract .
	manualset3
197345	4	416146	7	NULL	NULL	0	NULL	27 primiparae	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Urodynamic investigations including cystometry and electronic simultaneous urethro-cystometry were made in 27 primiparae between 2 and 5 days after delivery to assess possible effects of lumbar epidural analgesia on the function of the lower urinary tract .
	manualset3
197346	5	416146	7	NULL	NULL	0	NULL	2 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Urodynamic investigations including cystometry and electronic simultaneous urethro-cystometry were made in 27 primiparae between 2 and 5 days after delivery to assess possible effects of lumbar epidural analgesia on the function of the lower urinary tract .
	manualset3
197347	6	416146	7	NULL	NULL	0	NULL	5 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Urodynamic investigations including cystometry and electronic simultaneous urethro-cystometry were made in 27 primiparae between 2 and 5 days after delivery to assess possible effects of lumbar epidural analgesia on the function of the lower urinary tract .
	manualset3
197348	7	416146	7	NULL	NULL	0	NULL	delivery	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Urodynamic investigations including cystometry and electronic simultaneous urethro-cystometry were made in 27 primiparae between 2 and 5 days after delivery to assess possible effects of lumbar epidural analgesia on the function of the lower urinary tract .
	manualset3
197349	8	416146	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Urodynamic investigations including cystometry and electronic simultaneous urethro-cystometry were made in 27 primiparae between 2 and 5 days after delivery to assess possible effects of lumbar epidural analgesia on the function of the lower urinary tract .
	manualset3
197350	9	416146	7	NULL	NULL	0	NULL	lumbar epidural analgesia	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Urodynamic investigations including cystometry and electronic simultaneous urethro-cystometry were made in 27 primiparae between 2 and 5 days after delivery to assess possible effects of lumbar epidural analgesia on the function of the lower urinary tract .
	manualset3
197351	10	416146	7	NULL	NULL	0	NULL	function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Urodynamic investigations including cystometry and electronic simultaneous urethro-cystometry were made in 27 primiparae between 2 and 5 days after delivery to assess possible effects of lumbar epidural analgesia on the function of the lower urinary tract .
	manualset3
197352	11	416146	7	NULL	NULL	0	NULL	lower urinary tract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Urodynamic investigations including cystometry and electronic simultaneous urethro-cystometry were made in 27 primiparae between 2 and 5 days after delivery to assess possible effects of lumbar epidural analgesia on the function of the lower urinary tract .
	manualset3
197353	1	416147	7	NULL	NULL	0	NULL	Urokinase-type PA ( u-PA ) activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Urokinase-type PA ( u-PA ) activity was also identified in pre - and postexercise samples at an apparent mol wt of approximately 50 , 000 .
	manualset3
197354	2	416147	7	NULL	NULL	0	NULL	pre -exercise samples	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Urokinase-type PA ( u-PA ) activity was also identified in pre - and postexercise samples at an apparent mol wt of approximately 50 , 000 .
	manualset3
197355	3	416147	7	NULL	NULL	0	NULL	postexercise samples	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Urokinase-type PA ( u-PA ) activity was also identified in pre - and postexercise samples at an apparent mol wt of approximately 50 , 000 .
	manualset3
197356	4	416147	7	NULL	NULL	0	NULL	mol wt	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Urokinase-type PA ( u-PA ) activity was also identified in pre - and postexercise samples at an apparent mol wt of approximately 50 , 000 .
	manualset3
197357	5	416147	7	NULL	NULL	0	NULL	50 , 000	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Urokinase-type PA ( u-PA ) activity was also identified in pre - and postexercise samples at an apparent mol wt of approximately 50 , 000 .
	manualset3
197358	1	416148	7	NULL	NULL	0	NULL	Urokinase-type plasminogen activator	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Urokinase-type plasminogen activator and plasminogen activator inhibitors ( PAI-1 and PAI-2 ) in extracts of invasive cervical carcinoma and precursor lesions .
	manualset3
197359	2	416148	7	NULL	NULL	0	NULL	plasminogen activator inhibitors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Urokinase-type plasminogen activator and plasminogen activator inhibitors ( PAI-1 and PAI-2 ) in extracts of invasive cervical carcinoma and precursor lesions .
	manualset3
197360	3	416148	7	NULL	NULL	0	NULL	PAI-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Urokinase-type plasminogen activator and plasminogen activator inhibitors ( PAI-1 and PAI-2 ) in extracts of invasive cervical carcinoma and precursor lesions .
	manualset3
197361	4	416148	7	NULL	NULL	0	NULL	PAI-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Urokinase-type plasminogen activator and plasminogen activator inhibitors ( PAI-1 and PAI-2 ) in extracts of invasive cervical carcinoma and precursor lesions .
	manualset3
197362	5	416148	7	NULL	NULL	0	NULL	extracts	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Urokinase-type plasminogen activator and plasminogen activator inhibitors ( PAI-1 and PAI-2 ) in extracts of invasive cervical carcinoma and precursor lesions .
	manualset3
197363	6	416148	7	NULL	NULL	0	NULL	invasive cervical carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Urokinase-type plasminogen activator and plasminogen activator inhibitors ( PAI-1 and PAI-2 ) in extracts of invasive cervical carcinoma and precursor lesions .
	manualset3
197364	7	416148	7	NULL	NULL	0	NULL	precursor lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Urokinase-type plasminogen activator and plasminogen activator inhibitors ( PAI-1 and PAI-2 ) in extracts of invasive cervical carcinoma and precursor lesions .
	manualset3
197365	1	416149	7	NULL	NULL	NULL	NULL	rotensin II-induced endothelin-1 expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Urotensin II-induced endothelin-1 expression and cell proliferation via epidermal growth factor receptor transactivation in rat aortic smooth muscle cells .
	manualset3
197366	2	416149	7	NULL	NULL	0	NULL	cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Urotensin II-induced endothelin-1 expression and cell proliferation via epidermal growth factor receptor transactivation in rat aortic smooth muscle cells .
	manualset3
197367	3	416149	7	NULL	NULL	NULL	NULL	 epidermal growth factor receptor  transactivation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Urotensin II-induced endothelin-1 expression and cell proliferation via epidermal growth factor receptor transactivation in rat aortic smooth muscle cells .
	manualset3
197368	4	416149	7	NULL	NULL	0	NULL	rat aortic smooth muscle cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Urotensin II-induced endothelin-1 expression and cell proliferation via epidermal growth factor receptor transactivation in rat aortic smooth muscle cells .
	manualset3
197369	1	416150	7	NULL	NULL	0	NULL	Use-dependent block	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Use-dependent block of INa was also observed .
	manualset3
197370	2	416150	7	NULL	NULL	0	NULL	INa	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Use-dependent block of INa was also observed .
	manualset3
197371	1	416151	7	NULL	NULL	NULL	NULL	Use of A. niger-preferred codon usage	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of A. niger-preferred codon usage and lower A+T content in a synthetic gene ( GP-syn ) resulted in a significant improvement in the level of the GP mRNA and a dramatic increase in the quantity of GP protein produced such that it accounted for approximately 10 % of the total soluble protein .
	manualset3
197372	2	416151	7	NULL	NULL	0	NULL	lower A+T content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of A. niger-preferred codon usage and lower A+T content in a synthetic gene ( GP-syn ) resulted in a significant improvement in the level of the GP mRNA and a dramatic increase in the quantity of GP protein produced such that it accounted for approximately 10 % of the total soluble protein .
	manualset3
197373	3	416151	7	NULL	NULL	0	NULL	synthetic gene ( GP-syn ) 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of A. niger-preferred codon usage and lower A+T content in a synthetic gene ( GP-syn ) resulted in a significant improvement in the level of the GP mRNA and a dramatic increase in the quantity of GP protein produced such that it accounted for approximately 10 % of the total soluble protein .
	manualset3
197374	4	416151	7	NULL	NULL	0	NULL	 improvement 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of A. niger-preferred codon usage and lower A+T content in a synthetic gene ( GP-syn ) resulted in a significant improvement in the level of the GP mRNA and a dramatic increase in the quantity of GP protein produced such that it accounted for approximately 10 % of the total soluble protein .
	manualset3
197375	5	416151	7	NULL	NULL	0	NULL	level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of A. niger-preferred codon usage and lower A+T content in a synthetic gene ( GP-syn ) resulted in a significant improvement in the level of the GP mRNA and a dramatic increase in the quantity of GP protein produced such that it accounted for approximately 10 % of the total soluble protein .
	manualset3
197376	6	416151	7	NULL	NULL	0	NULL	GP mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of A. niger-preferred codon usage and lower A+T content in a synthetic gene ( GP-syn ) resulted in a significant improvement in the level of the GP mRNA and a dramatic increase in the quantity of GP protein produced such that it accounted for approximately 10 % of the total soluble protein .
	manualset3
197377	7	416151	7	NULL	NULL	0	NULL	dramatic increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of A. niger-preferred codon usage and lower A+T content in a synthetic gene ( GP-syn ) resulted in a significant improvement in the level of the GP mRNA and a dramatic increase in the quantity of GP protein produced such that it accounted for approximately 10 % of the total soluble protein .
	manualset3
197378	8	416151	7	NULL	NULL	0	NULL	quantity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of A. niger-preferred codon usage and lower A+T content in a synthetic gene ( GP-syn ) resulted in a significant improvement in the level of the GP mRNA and a dramatic increase in the quantity of GP protein produced such that it accounted for approximately 10 % of the total soluble protein .
	manualset3
197379	9	416151	7	NULL	NULL	0	NULL	GP protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of A. niger-preferred codon usage and lower A+T content in a synthetic gene ( GP-syn ) resulted in a significant improvement in the level of the GP mRNA and a dramatic increase in the quantity of GP protein produced such that it accounted for approximately 10 % of the total soluble protein .
	manualset3
197380	10	416151	7	NULL	NULL	0	NULL	10 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of A. niger-preferred codon usage and lower A+T content in a synthetic gene ( GP-syn ) resulted in a significant improvement in the level of the GP mRNA and a dramatic increase in the quantity of GP protein produced such that it accounted for approximately 10 % of the total soluble protein .
	manualset3
197381	11	416151	7	NULL	NULL	0	NULL	total soluble protein	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of A. niger-preferred codon usage and lower A+T content in a synthetic gene ( GP-syn ) resulted in a significant improvement in the level of the GP mRNA and a dramatic increase in the quantity of GP protein produced such that it accounted for approximately 10 % of the total soluble protein .
	manualset3
197382	1	416152	7	NULL	NULL	NULL	NULL	Use of RNA interference	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of RNA interference resulted in the generation of stable cell lines that express constitutively low levels of vimentin .
	manualset3
197383	2	416152	7	NULL	NULL	0	NULL	generation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of RNA interference resulted in the generation of stable cell lines that express constitutively low levels of vimentin .
	manualset3
197384	3	416152	7	NULL	NULL	0	NULL	 stable cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of RNA interference resulted in the generation of stable cell lines that express constitutively low levels of vimentin .
	manualset3
197385	4	416152	7	NULL	NULL	0	NULL	low levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of RNA interference resulted in the generation of stable cell lines that express constitutively low levels of vimentin .
	manualset3
197386	5	416152	7	NULL	NULL	0	NULL	vimentin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of RNA interference resulted in the generation of stable cell lines that express constitutively low levels of vimentin .
	manualset3
197387	1	416153	7	NULL	NULL	NULL	NULL	Use of a laryngeal mask	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of a laryngeal mask in acute airway obstruction after carotid endarterectomy .
	manualset3
197388	2	416153	7	NULL	NULL	0	NULL	acute airway obstruction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of a laryngeal mask in acute airway obstruction after carotid endarterectomy .
	manualset3
197389	3	416153	7	NULL	NULL	0	NULL	 carotid endarterectomy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of a laryngeal mask in acute airway obstruction after carotid endarterectomy .
	manualset3
197390	1	416154	7	NULL	NULL	NULL	NULL	Use of a zwitterionic detergent	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of a zwitterionic detergent for the restoration of the antibody-binding capacity of electroblotted meningococcal outer membrane proteins .
	manualset3
197391	2	416154	7	NULL	NULL	NULL	NULL	 restoration	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of a zwitterionic detergent for the restoration of the antibody-binding capacity of electroblotted meningococcal outer membrane proteins .
	manualset3
197392	3	416154	7	NULL	NULL	0	NULL	antibody-binding capacity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of a zwitterionic detergent for the restoration of the antibody-binding capacity of electroblotted meningococcal outer membrane proteins .
	manualset3
197393	4	416154	7	NULL	NULL	0	NULL	electroblotted meningococcal outer membrane proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of a zwitterionic detergent for the restoration of the antibody-binding capacity of electroblotted meningococcal outer membrane proteins .
	manualset3
197394	1	416155	7	NULL	NULL	NULL	NULL	Use of arm veins	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of arm veins for lower extremity arterial bypass -- results , anatomical features and technical considerations .
	manualset3
197395	2	416155	7	NULL	NULL	0	NULL	lower extremity arterial bypass	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of arm veins for lower extremity arterial bypass -- results , anatomical features and technical considerations .
	manualset3
197396	3	416155	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of arm veins for lower extremity arterial bypass -- results , anatomical features and technical considerations .
	manualset3
197397	4	416155	7	NULL	NULL	0	NULL	anatomical features 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of arm veins for lower extremity arterial bypass -- results , anatomical features and technical considerations .
	manualset3
197398	5	416155	7	NULL	NULL	0	NULL	technical considerations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of arm veins for lower extremity arterial bypass -- results , anatomical features and technical considerations .
	manualset3
197399	1	416156	7	NULL	NULL	NULL	NULL	 Use of assessment tools	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of assessment tools that quantify the primary risk factors for the development of pressure ulcers is helpful in predicting and preventing compromise of tissue .
	manualset3
197400	2	416156	7	NULL	NULL	0	NULL	primary risk factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of assessment tools that quantify the primary risk factors for the development of pressure ulcers is helpful in predicting and preventing compromise of tissue .
	manualset3
197401	3	416156	7	NULL	NULL	0	NULL	 development	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of assessment tools that quantify the primary risk factors for the development of pressure ulcers is helpful in predicting and preventing compromise of tissue .
	manualset3
197402	4	416156	7	NULL	NULL	0	NULL	pressure ulcers	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of assessment tools that quantify the primary risk factors for the development of pressure ulcers is helpful in predicting and preventing compromise of tissue .
	manualset3
197403	5	416156	7	NULL	NULL	0	NULL	 tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of assessment tools that quantify the primary risk factors for the development of pressure ulcers is helpful in predicting and preventing compromise of tissue .
	manualset3
197404	1	416157	7	NULL	NULL	NULL	NULL	Use of  atorvastatin	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of atorvastatin in systemic lupus erythematosus in children and adolescents .
	manualset3
197405	2	416157	7	NULL	NULL	0	NULL	 systemic lupus erythematosus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of atorvastatin in systemic lupus erythematosus in children and adolescents .
	manualset3
197406	3	416157	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of atorvastatin in systemic lupus erythematosus in children and adolescents .
	manualset3
197407	4	416157	7	NULL	NULL	0	NULL	adolescents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of atorvastatin in systemic lupus erythematosus in children and adolescents .
	manualset3
197408	1	416158	7	NULL	NULL	NULL	NULL	Use of cardiac computed tomography	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of cardiac computed tomography prior to percutaneous coronary sinus device placement for the treatment of mitral regurgitation .
	manualset3
197409	2	416158	7	NULL	NULL	0	NULL	percutaneous coronary sinus device placement	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of cardiac computed tomography prior to percutaneous coronary sinus device placement for the treatment of mitral regurgitation .
	manualset3
197410	3	416158	7	NULL	NULL	0	NULL	 treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of cardiac computed tomography prior to percutaneous coronary sinus device placement for the treatment of mitral regurgitation .
	manualset3
197411	4	416158	7	NULL	NULL	0	NULL	mitral regurgitation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of cardiac computed tomography prior to percutaneous coronary sinus device placement for the treatment of mitral regurgitation .
	manualset3
197412	1	416159	7	NULL	NULL	NULL	NULL	Use of complementary therapy 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of complementary therapy by adolescents with asthma .
	manualset3
197413	2	416159	7	NULL	NULL	0	NULL	adolescents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of complementary therapy by adolescents with asthma .
	manualset3
197414	3	416159	7	NULL	NULL	0	NULL	asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of complementary therapy by adolescents with asthma .
	manualset3
197415	1	416160	7	NULL	NULL	NULL	NULL	Use of cyclophosphamide	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of cyclophosphamide as a positive control in dominant lethal and micronucleus assays .
	manualset3
197416	2	416160	7	NULL	NULL	0	NULL	 positive control 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of cyclophosphamide as a positive control in dominant lethal and micronucleus assays .
	manualset3
197417	3	416160	7	NULL	NULL	NULL	NULL	dominant lethal assays	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of cyclophosphamide as a positive control in dominant lethal and micronucleus assays .
	manualset3
197418	4	416160	7	NULL	NULL	NULL	NULL	micronucleus assays	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of cyclophosphamide as a positive control in dominant lethal and micronucleus assays .
	manualset3
197419	1	416161	7	NULL	NULL	0	NULL	treatments	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After the treatments , blood samples were collected at 0 , 1 , 2 , 4 , 6 , 8 , 12 , 24 and 48 h. Oxidative stress parameters were determined by ELISA , while serum organ damage markers were measured by autoanalyser .
	manualset3
197420	2	416161	7	NULL	NULL	0	NULL	blood samples	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After the treatments , blood samples were collected at 0 , 1 , 2 , 4 , 6 , 8 , 12 , 24 and 48 h. Oxidative stress parameters were determined by ELISA , while serum organ damage markers were measured by autoanalyser .
	manualset3
197421	3	416161	7	NULL	NULL	0	NULL	0 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After the treatments , blood samples were collected at 0 , 1 , 2 , 4 , 6 , 8 , 12 , 24 and 48 h. Oxidative stress parameters were determined by ELISA , while serum organ damage markers were measured by autoanalyser .
	manualset3
197422	4	416161	7	NULL	NULL	0	NULL	1 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After the treatments , blood samples were collected at 0 , 1 , 2 , 4 , 6 , 8 , 12 , 24 and 48 h. Oxidative stress parameters were determined by ELISA , while serum organ damage markers were measured by autoanalyser .
	manualset3
197423	5	416161	7	NULL	NULL	0	NULL	2 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After the treatments , blood samples were collected at 0 , 1 , 2 , 4 , 6 , 8 , 12 , 24 and 48 h. Oxidative stress parameters were determined by ELISA , while serum organ damage markers were measured by autoanalyser .
	manualset3
197424	6	416161	7	NULL	NULL	0	NULL	4 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After the treatments , blood samples were collected at 0 , 1 , 2 , 4 , 6 , 8 , 12 , 24 and 48 h. Oxidative stress parameters were determined by ELISA , while serum organ damage markers were measured by autoanalyser .
	manualset3
197425	7	416161	7	NULL	NULL	0	NULL	6 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After the treatments , blood samples were collected at 0 , 1 , 2 , 4 , 6 , 8 , 12 , 24 and 48 h. Oxidative stress parameters were determined by ELISA , while serum organ damage markers were measured by autoanalyser .
	manualset3
197426	8	416161	7	NULL	NULL	0	NULL	8 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After the treatments , blood samples were collected at 0 , 1 , 2 , 4 , 6 , 8 , 12 , 24 and 48 h. Oxidative stress parameters were determined by ELISA , while serum organ damage markers were measured by autoanalyser .
	manualset3
197427	9	416161	7	NULL	NULL	0	NULL	12 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After the treatments , blood samples were collected at 0 , 1 , 2 , 4 , 6 , 8 , 12 , 24 and 48 h. Oxidative stress parameters were determined by ELISA , while serum organ damage markers were measured by autoanalyser .
	manualset3
197428	10	416161	7	NULL	NULL	0	NULL	24 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After the treatments , blood samples were collected at 0 , 1 , 2 , 4 , 6 , 8 , 12 , 24 and 48 h. Oxidative stress parameters were determined by ELISA , while serum organ damage markers were measured by autoanalyser .
	manualset3
197429	11	416161	7	NULL	NULL	0	NULL	48 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After the treatments , blood samples were collected at 0 , 1 , 2 , 4 , 6 , 8 , 12 , 24 and 48 h. Oxidative stress parameters were determined by ELISA , while serum organ damage markers were measured by autoanalyser .
	manualset3
197430	12	416161	7	NULL	NULL	0	NULL	 Oxidative stress parameters	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	After the treatments , blood samples were collected at 0 , 1 , 2 , 4 , 6 , 8 , 12 , 24 and 48 h. Oxidative stress parameters were determined by ELISA , while serum organ damage markers were measured by autoanalyser .
	manualset3
197431	13	416161	7	NULL	NULL	0	NULL	ELISA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After the treatments , blood samples were collected at 0 , 1 , 2 , 4 , 6 , 8 , 12 , 24 and 48 h. Oxidative stress parameters were determined by ELISA , while serum organ damage markers were measured by autoanalyser .
	manualset3
197432	14	416161	7	NULL	NULL	0	NULL	serum organ damage markers	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	After the treatments , blood samples were collected at 0 , 1 , 2 , 4 , 6 , 8 , 12 , 24 and 48 h. Oxidative stress parameters were determined by ELISA , while serum organ damage markers were measured by autoanalyser .
	manualset3
197433	15	416161	7	NULL	NULL	NULL	NULL	autoanalyser	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After the treatments , blood samples were collected at 0 , 1 , 2 , 4 , 6 , 8 , 12 , 24 and 48 h. Oxidative stress parameters were determined by ELISA , while serum organ damage markers were measured by autoanalyser .
	manualset3
197434	1	416162	7	NULL	NULL	NULL	NULL	exercise thallium scintigraphy 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of exercise thallium scintigraphy to assess extent of ischaemic myocardium in patients with left anterior descending artery disease .
	manualset3
197435	2	416162	7	NULL	NULL	0	NULL	 ischaemic myocardium	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of exercise thallium scintigraphy to assess extent of ischaemic myocardium in patients with left anterior descending artery disease .
	manualset3
197436	3	416162	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of exercise thallium scintigraphy to assess extent of ischaemic myocardium in patients with left anterior descending artery disease .
	manualset3
197437	4	416162	7	NULL	NULL	0	NULL	left anterior descending artery disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of exercise thallium scintigraphy to assess extent of ischaemic myocardium in patients with left anterior descending artery disease .
	manualset3
200262	5	416162	7	NULL	NULL	0	NULL	extent	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of exercise thallium scintigraphy to assess extent of ischaemic myocardium in patients with left anterior descending artery disease .
	manualset3
203033	6	416162	7	NULL	NULL	0	NULL	Use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of exercise thallium scintigraphy to assess extent of ischaemic myocardium in patients with left anterior descending artery disease .
	manualset3
197438	1	416163	7	NULL	NULL	NULL	NULL	exit examinations	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of exit examinations : a criterion for graduation ?
	manualset3
197439	2	416163	7	NULL	NULL	0	NULL	 criterion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of exit examinations : a criterion for graduation ?
	manualset3
197440	3	416163	7	NULL	NULL	0	NULL	 graduation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of exit examinations : a criterion for graduation ?
	manualset3
203034	4	416163	7	NULL	NULL	0	NULL	Use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of exit examinations : a criterion for graduation ?
	manualset3
197441	1	416164	7	NULL	NULL	NULL	NULL	 glycogen phosphorylase BB measurement 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of glycogen phosphorylase BB measurement with POCT in the diagnosis of acute coronary syndromes .
	manualset3
197442	2	416164	7	NULL	NULL	0	NULL	POCT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of glycogen phosphorylase BB measurement with POCT in the diagnosis of acute coronary syndromes .
	manualset3
197443	3	416164	7	NULL	NULL	0	NULL	 diagnosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of glycogen phosphorylase BB measurement with POCT in the diagnosis of acute coronary syndromes .
	manualset3
197444	4	416164	7	NULL	NULL	0	NULL	acute coronary syndromes 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of glycogen phosphorylase BB measurement with POCT in the diagnosis of acute coronary syndromes .
	manualset3
203035	5	416164	7	NULL	NULL	0	NULL	Use	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of glycogen phosphorylase BB measurement with POCT in the diagnosis of acute coronary syndromes .
	manualset3
197445	1	416165	7	NULL	NULL	NULL	NULL	 high density antibody arrays	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of high density antibody arrays to validate and discover cancer serum biomarkers .
	manualset3
197446	2	416165	7	NULL	NULL	0	NULL	 cancer serum biomarkers	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of high density antibody arrays to validate and discover cancer serum biomarkers .
	manualset3
203036	3	416165	7	NULL	NULL	0	NULL	Use	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of high density antibody arrays to validate and discover cancer serum biomarkers .
	manualset3
197447	1	416166	7	NULL	NULL	NULL	NULL	Use of immobilized proteinases	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of immobilized proteinases and peptidases to study structural changes in proteins .
	manualset3
197448	2	416166	7	NULL	NULL	NULL	NULL	Use of peptidases	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of immobilized proteinases and peptidases to study structural changes in proteins .
	manualset3
197449	3	416166	7	NULL	NULL	0	NULL	structural changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of immobilized proteinases and peptidases to study structural changes in proteins .
	manualset3
197450	4	416166	7	NULL	NULL	0	NULL	proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of immobilized proteinases and peptidases to study structural changes in proteins .
	manualset3
197451	1	416167	7	NULL	NULL	NULL	NULL	intravenous diazepam 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of intravenous diazepam in acute skeletal muscle spasm .
	manualset3
197452	2	416167	7	NULL	NULL	0	NULL	acute skeletal muscle spasm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of intravenous diazepam in acute skeletal muscle spasm .
	manualset3
203037	3	416167	7	NULL	NULL	0	NULL	Use 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of intravenous diazepam in acute skeletal muscle spasm .
	manualset3
197453	1	416168	7	NULL	NULL	NULL	NULL	magnification	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of magnification , a bloodless field , injection of a relatively large volume of local anesthetic ( 10 to 12 cc ) , knowledge of regional anatomy , and careful surgical technique decrease the risk of nerve injury .
	manualset3
197454	2	416168	7	NULL	NULL	0	NULL	bloodless field	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of magnification , a bloodless field , injection of a relatively large volume of local anesthetic ( 10 to 12 cc ) , knowledge of regional anatomy , and careful surgical technique decrease the risk of nerve injury .
	manualset3
197455	3	416168	7	NULL	NULL	0	NULL	 injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of magnification , a bloodless field , injection of a relatively large volume of local anesthetic ( 10 to 12 cc ) , knowledge of regional anatomy , and careful surgical technique decrease the risk of nerve injury .
	manualset3
197456	4	416168	7	NULL	NULL	0	NULL	 relatively large volume	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of magnification , a bloodless field , injection of a relatively large volume of local anesthetic ( 10 to 12 cc ) , knowledge of regional anatomy , and careful surgical technique decrease the risk of nerve injury .
	manualset3
197457	5	416168	7	NULL	NULL	0	NULL	 local anesthetic 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of magnification , a bloodless field , injection of a relatively large volume of local anesthetic ( 10 to 12 cc ) , knowledge of regional anatomy , and careful surgical technique decrease the risk of nerve injury .
	manualset3
197458	6	416168	7	NULL	NULL	0	NULL	10 to 12 cc	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of magnification , a bloodless field , injection of a relatively large volume of local anesthetic ( 10 to 12 cc ) , knowledge of regional anatomy , and careful surgical technique decrease the risk of nerve injury .
	manualset3
197459	7	416168	7	NULL	NULL	0	NULL	knowledge	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of magnification , a bloodless field , injection of a relatively large volume of local anesthetic ( 10 to 12 cc ) , knowledge of regional anatomy , and careful surgical technique decrease the risk of nerve injury .
	manualset3
197460	8	416168	7	NULL	NULL	0	NULL	regional anatomy	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of magnification , a bloodless field , injection of a relatively large volume of local anesthetic ( 10 to 12 cc ) , knowledge of regional anatomy , and careful surgical technique decrease the risk of nerve injury .
	manualset3
197461	9	416168	7	NULL	NULL	0	NULL	surgical technique	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of magnification , a bloodless field , injection of a relatively large volume of local anesthetic ( 10 to 12 cc ) , knowledge of regional anatomy , and careful surgical technique decrease the risk of nerve injury .
	manualset3
197462	10	416168	7	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of magnification , a bloodless field , injection of a relatively large volume of local anesthetic ( 10 to 12 cc ) , knowledge of regional anatomy , and careful surgical technique decrease the risk of nerve injury .
	manualset3
197463	11	416168	7	NULL	NULL	0	NULL	nerve injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of magnification , a bloodless field , injection of a relatively large volume of local anesthetic ( 10 to 12 cc ) , knowledge of regional anatomy , and careful surgical technique decrease the risk of nerve injury .
	manualset3
203038	12	416168	7	NULL	NULL	0	NULL	Use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of magnification , a bloodless field , injection of a relatively large volume of local anesthetic ( 10 to 12 cc ) , knowledge of regional anatomy , and careful surgical technique decrease the risk of nerve injury .
	manualset3
197464	1	416169	7	NULL	NULL	NULL	NULL	 niacin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of niacin in low doses usually leads to few adverse drug reactions ( ADRs ) ; however , at larger doses , niacin can cause skin flushing , itching , and occasionally more serious effects .
	manualset3
197465	2	416169	7	NULL	NULL	0	NULL	 low doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of niacin in low doses usually leads to few adverse drug reactions ( ADRs ) ; however , at larger doses , niacin can cause skin flushing , itching , and occasionally more serious effects .
	manualset3
197466	3	416169	7	NULL	NULL	0	NULL	adverse drug reactions ( ADRs )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of niacin in low doses usually leads to few adverse drug reactions ( ADRs ) ; however , at larger doses , niacin can cause skin flushing , itching , and occasionally more serious effects .
	manualset3
197467	4	416169	7	NULL	NULL	0	NULL	 larger doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of niacin in low doses usually leads to few adverse drug reactions ( ADRs ) ; however , at larger doses , niacin can cause skin flushing , itching , and occasionally more serious effects .
	manualset3
197468	5	416169	7	NULL	NULL	0	NULL	niacin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of niacin in low doses usually leads to few adverse drug reactions ( ADRs ) ; however , at larger doses , niacin can cause skin flushing , itching , and occasionally more serious effects .
	manualset3
197469	6	416169	7	NULL	NULL	0	NULL	skin flushing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of niacin in low doses usually leads to few adverse drug reactions ( ADRs ) ; however , at larger doses , niacin can cause skin flushing , itching , and occasionally more serious effects .
	manualset3
197470	7	416169	7	NULL	NULL	0	NULL	 itching	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of niacin in low doses usually leads to few adverse drug reactions ( ADRs ) ; however , at larger doses , niacin can cause skin flushing , itching , and occasionally more serious effects .
	manualset3
197471	8	416169	7	NULL	NULL	0	NULL	 serious effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of niacin in low doses usually leads to few adverse drug reactions ( ADRs ) ; however , at larger doses , niacin can cause skin flushing , itching , and occasionally more serious effects .
	manualset3
203039	9	416169	7	NULL	NULL	0	NULL	Use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of niacin in low doses usually leads to few adverse drug reactions ( ADRs ) ; however , at larger doses , niacin can cause skin flushing , itching , and occasionally more serious effects .
	manualset3
197472	1	416170	7	NULL	NULL	NULL	NULL	 occupational health setting	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of occupational health setting for nursing student experiences .
	manualset3
197473	2	416170	7	NULL	NULL	0	NULL	 nursing student experiences 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of occupational health setting for nursing student experiences .
	manualset3
203040	3	416170	7	NULL	NULL	0	NULL	Use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of occupational health setting for nursing student experiences .
	manualset3
197474	1	416171	7	NULL	NULL	NULL	NULL	 pH-stat blood gas management	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of pH-stat blood gas management has been shown to increase cerebral blood flow during cooling .
	manualset3
197475	2	416171	7	NULL	NULL	0	NULL	cerebral blood flow	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of pH-stat blood gas management has been shown to increase cerebral blood flow during cooling .
	manualset3
197476	3	416171	7	NULL	NULL	0	NULL	cooling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of pH-stat blood gas management has been shown to increase cerebral blood flow during cooling .
	manualset3
203041	4	416171	7	NULL	NULL	0	NULL	Use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of pH-stat blood gas management has been shown to increase cerebral blood flow during cooling .
	manualset3
197477	1	416172	7	NULL	NULL	0	NULL	 war	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After the war , elephant densities were relatively higher in the center of the park where they were better protected , suggesting that this area may have acted as a refuge .
	manualset3
197478	2	416172	7	NULL	NULL	0	NULL	elephant densities	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After the war , elephant densities were relatively higher in the center of the park where they were better protected , suggesting that this area may have acted as a refuge .
	manualset3
197479	3	416172	7	NULL	NULL	0	NULL	center of the park	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	After the war , elephant densities were relatively higher in the center of the park where they were better protected , suggesting that this area may have acted as a refuge .
	manualset3
197480	4	416172	7	NULL	NULL	0	NULL	area 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	After the war , elephant densities were relatively higher in the center of the park where they were better protected , suggesting that this area may have acted as a refuge .
	manualset3
197481	5	416172	7	NULL	NULL	0	NULL	 refuge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After the war , elephant densities were relatively higher in the center of the park where they were better protected , suggesting that this area may have acted as a refuge .
	manualset3
197482	1	416173	7	NULL	NULL	NULL	NULL	surface electromyogram	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of surface electromyogram as a measure of dynamic force in human limb muscles .
	manualset3
197483	2	416173	7	NULL	NULL	0	NULL	dynamic force	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of surface electromyogram as a measure of dynamic force in human limb muscles .
	manualset3
197484	3	416173	7	NULL	NULL	0	NULL	human limb muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of surface electromyogram as a measure of dynamic force in human limb muscles .
	manualset3
203042	4	416173	7	NULL	NULL	0	NULL	Use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of surface electromyogram as a measure of dynamic force in human limb muscles .
	manualset3
197485	1	416174	7	NULL	NULL	NULL	NULL	 text messaging 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of text messaging to audit early clinical outcome following vasectomy in primary care .
	manualset3
197486	2	416174	7	NULL	NULL	0	NULL	early clinical outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of text messaging to audit early clinical outcome following vasectomy in primary care .
	manualset3
197487	3	416174	7	NULL	NULL	0	NULL	vasectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of text messaging to audit early clinical outcome following vasectomy in primary care .
	manualset3
197488	4	416174	7	NULL	NULL	0	NULL	primary care	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of text messaging to audit early clinical outcome following vasectomy in primary care .
	manualset3
203043	5	416174	7	NULL	NULL	0	NULL	Use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of text messaging to audit early clinical outcome following vasectomy in primary care .
	manualset3
197489	1	416175	7	NULL	NULL	NULL	NULL	 DNA flow-thru chip	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of the DNA flow-thru chip , a three-dimensional biochip , for typing and subtyping of influenza viruses .
	manualset3
197490	2	416175	7	NULL	NULL	0	NULL	three-dimensional biochip	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of the DNA flow-thru chip , a three-dimensional biochip , for typing and subtyping of influenza viruses .
	manualset3
197491	3	416175	7	NULL	NULL	0	NULL	typing 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of the DNA flow-thru chip , a three-dimensional biochip , for typing and subtyping of influenza viruses .
	manualset3
197492	4	416175	7	NULL	NULL	0	NULL	subtyping	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of the DNA flow-thru chip , a three-dimensional biochip , for typing and subtyping of influenza viruses .
	manualset3
197493	5	416175	7	NULL	NULL	0	NULL	influenza viruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of the DNA flow-thru chip , a three-dimensional biochip , for typing and subtyping of influenza viruses .
	manualset3
203044	6	416175	7	NULL	NULL	0	NULL	Use	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of the DNA flow-thru chip , a three-dimensional biochip , for typing and subtyping of influenza viruses .
	manualset3
197494	1	416176	7	NULL	NULL	NULL	NULL	 unproven drugs	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of unproven and unapproved drugs to treat cocaine addiction .
	manualset3
197495	2	416176	7	NULL	NULL	NULL	NULL	unapproved drugs	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of unproven and unapproved drugs to treat cocaine addiction .
	manualset3
197496	3	416176	7	NULL	NULL	0	NULL	cocaine addiction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of unproven and unapproved drugs to treat cocaine addiction .
	manualset3
203045	4	416176	7	NULL	NULL	0	NULL	Use	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of unproven and unapproved drugs to treat cocaine addiction .
	manualset3
197497	1	416177	7	NULL	NULL	NULL	NULL	 written material 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of written material in learning self-control of premature ejaculation .
	manualset3
197498	2	416177	7	NULL	NULL	0	NULL	learning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of written material in learning self-control of premature ejaculation .
	manualset3
197499	3	416177	7	NULL	NULL	NULL	NULL	self-control	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of written material in learning self-control of premature ejaculation .
	manualset3
197500	4	416177	7	NULL	NULL	0	NULL	 premature ejaculation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of written material in learning self-control of premature ejaculation .
	manualset3
203046	5	416177	7	NULL	NULL	0	NULL	Use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of written material in learning self-control of premature ejaculation .
	manualset3
197501	1	416178	7	NULL	NULL	NULL	NULL	polyethylene terephthalate bottles ( PET )	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Used polyethylene terephthalate bottles ( PET ) dumped indiscriminately onto bare lands and water bodies constitute an eyesore .
	manualset3
197502	2	416178	7	NULL	NULL	0	NULL	 bare lands	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Used polyethylene terephthalate bottles ( PET ) dumped indiscriminately onto bare lands and water bodies constitute an eyesore .
	manualset3
197503	3	416178	7	NULL	NULL	0	NULL	water bodies 	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Used polyethylene terephthalate bottles ( PET ) dumped indiscriminately onto bare lands and water bodies constitute an eyesore .
	manualset3
197504	4	416178	7	NULL	NULL	NULL	NULL	eyesore	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Used polyethylene terephthalate bottles ( PET ) dumped indiscriminately onto bare lands and water bodies constitute an eyesore .
	manualset3
197505	1	416179	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After this , the addition of the compound in the absence of light did not produce any response .
	manualset3
197506	2	416179	7	NULL	NULL	0	NULL	compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After this , the addition of the compound in the absence of light did not produce any response .
	manualset3
197507	3	416179	7	NULL	NULL	0	NULL	light	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	After this , the addition of the compound in the absence of light did not produce any response .
	manualset3
197508	4	416179	7	NULL	NULL	0	NULL	 response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After this , the addition of the compound in the absence of light did not produce any response .
	manualset3
197509	1	416180	7	NULL	NULL	NULL	NULL	cardiac iodine-123 meta-iodobenzylguanidine imaging	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Usefulness of cardiac iodine-123 meta-iodobenzylguanidine imaging to improve prognostic power of Seattle heart failure model in patients with chronic heart failure .
	manualset3
197510	2	416180	7	NULL	NULL	0	NULL	 prognostic power	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Usefulness of cardiac iodine-123 meta-iodobenzylguanidine imaging to improve prognostic power of Seattle heart failure model in patients with chronic heart failure .
	manualset3
197511	3	416180	7	NULL	NULL	0	NULL	Seattle heart failure model 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Usefulness of cardiac iodine-123 meta-iodobenzylguanidine imaging to improve prognostic power of Seattle heart failure model in patients with chronic heart failure .
	manualset3
197512	4	416180	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Usefulness of cardiac iodine-123 meta-iodobenzylguanidine imaging to improve prognostic power of Seattle heart failure model in patients with chronic heart failure .
	manualset3
197513	5	416180	7	NULL	NULL	0	NULL	chronic heart failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Usefulness of cardiac iodine-123 meta-iodobenzylguanidine imaging to improve prognostic power of Seattle heart failure model in patients with chronic heart failure .
	manualset3
203047	6	416180	7	NULL	NULL	0	NULL	Usefulness	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Usefulness of cardiac iodine-123 meta-iodobenzylguanidine imaging to improve prognostic power of Seattle heart failure model in patients with chronic heart failure .
	manualset3
197514	1	416181	7	NULL	NULL	0	NULL	User-based estimation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	User-based estimation of intima-media thickness ( IMT ) of carotid arteries leads to subjectivity in its decision support systems , while being used as a cardiovascular risk marker .
	manualset3
197515	2	416181	7	NULL	NULL	0	NULL	intima-media thickness ( IMT )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	User-based estimation of intima-media thickness ( IMT ) of carotid arteries leads to subjectivity in its decision support systems , while being used as a cardiovascular risk marker .
	manualset3
197516	3	416181	7	NULL	NULL	0	NULL	carotid arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	User-based estimation of intima-media thickness ( IMT ) of carotid arteries leads to subjectivity in its decision support systems , while being used as a cardiovascular risk marker .
	manualset3
197517	4	416181	7	NULL	NULL	0	NULL	decision support systems	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	User-based estimation of intima-media thickness ( IMT ) of carotid arteries leads to subjectivity in its decision support systems , while being used as a cardiovascular risk marker .
	manualset3
197518	5	416181	7	NULL	NULL	0	NULL	 cardiovascular risk marker	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	User-based estimation of intima-media thickness ( IMT ) of carotid arteries leads to subjectivity in its decision support systems , while being used as a cardiovascular risk marker .
	manualset3
197519	1	416182	7	NULL	NULL	0	NULL	Users	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Users of oral contraceptives had an age-adjusted risk of ovarian cancer developing of 0.6 relative to those who had never used them ( 95 % confidence interval , 0.4 to 0.9 ) .
	manualset3
197520	2	416182	7	NULL	NULL	0	NULL	oral contraceptives	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Users of oral contraceptives had an age-adjusted risk of ovarian cancer developing of 0.6 relative to those who had never used them ( 95 % confidence interval , 0.4 to 0.9 ) .
	manualset3
197521	3	416182	7	NULL	NULL	0	NULL	age-adjusted risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Users of oral contraceptives had an age-adjusted risk of ovarian cancer developing of 0.6 relative to those who had never used them ( 95 % confidence interval , 0.4 to 0.9 ) .
	manualset3
197522	4	416182	7	NULL	NULL	0	NULL	ovarian cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Users of oral contraceptives had an age-adjusted risk of ovarian cancer developing of 0.6 relative to those who had never used them ( 95 % confidence interval , 0.4 to 0.9 ) .
	manualset3
197523	5	416182	7	NULL	NULL	0	NULL	 0.6	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Users of oral contraceptives had an age-adjusted risk of ovarian cancer developing of 0.6 relative to those who had never used them ( 95 % confidence interval , 0.4 to 0.9 ) .
	manualset3
197524	6	416182	7	NULL	NULL	0	NULL	95 % confidence interval	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Users of oral contraceptives had an age-adjusted risk of ovarian cancer developing of 0.6 relative to those who had never used them ( 95 % confidence interval , 0.4 to 0.9 ) .
	manualset3
197525	7	416182	7	NULL	NULL	0	NULL	0.4 to 0.9	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Users of oral contraceptives had an age-adjusted risk of ovarian cancer developing of 0.6 relative to those who had never used them ( 95 % confidence interval , 0.4 to 0.9 ) .
	manualset3
197526	1	416183	7	NULL	NULL	0	NULL	Users	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Users should fully understand the risks and benefits before switching from the public switched telephone network .
	manualset3
197527	2	416183	7	NULL	NULL	0	NULL	risks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Users should fully understand the risks and benefits before switching from the public switched telephone network .
	manualset3
197528	3	416183	7	NULL	NULL	0	NULL	benefits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Users should fully understand the risks and benefits before switching from the public switched telephone network .
	manualset3
197529	4	416183	7	NULL	NULL	0	NULL	switching	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Users should fully understand the risks and benefits before switching from the public switched telephone network .
	manualset3
197530	5	416183	7	NULL	NULL	0	NULL	public switched telephone network	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Users should fully understand the risks and benefits before switching from the public switched telephone network .
	manualset3
197531	1	416184	7	NULL	NULL	0	NULL	vaccinia virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Uses of vaccinia virus in vaccine delivery .
	manualset3
197532	2	416184	7	NULL	NULL	0	NULL	 vaccine delivery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Uses of vaccinia virus in vaccine delivery .
	manualset3
203048	3	416184	7	NULL	NULL	0	NULL	Uses	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Uses of vaccinia virus in vaccine delivery .
	manualset3
197533	1	416185	7	NULL	NULL	0	NULL	0.45 M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Using 0.45 M PC 88 A , extraction isotherm was obtained at an aqueous-to-organic ( A : O ) phase ratio of 1 : 1 -3 and O : A ratio of 1 : 1 -5 , which predicted possible separation of Al in 2 stages at A/O ratio of 2 .
	manualset3
197534	2	416185	7	NULL	NULL	0	NULL	PC 88 A	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using 0.45 M PC 88 A , extraction isotherm was obtained at an aqueous-to-organic ( A : O ) phase ratio of 1 : 1 -3 and O : A ratio of 1 : 1 -5 , which predicted possible separation of Al in 2 stages at A/O ratio of 2 .
	manualset3
197535	3	416185	7	NULL	NULL	0	NULL	extraction isotherm	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Using 0.45 M PC 88 A , extraction isotherm was obtained at an aqueous-to-organic ( A : O ) phase ratio of 1 : 1 -3 and O : A ratio of 1 : 1 -5 , which predicted possible separation of Al in 2 stages at A/O ratio of 2 .
	manualset3
197536	4	416185	7	NULL	NULL	0	NULL	aqueous-to-organic ( A : O ) phase ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using 0.45 M PC 88 A , extraction isotherm was obtained at an aqueous-to-organic ( A : O ) phase ratio of 1 : 1 -3 and O : A ratio of 1 : 1 -5 , which predicted possible separation of Al in 2 stages at A/O ratio of 2 .
	manualset3
197537	5	416185	7	NULL	NULL	0	NULL	1 : 1 -3	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using 0.45 M PC 88 A , extraction isotherm was obtained at an aqueous-to-organic ( A : O ) phase ratio of 1 : 1 -3 and O : A ratio of 1 : 1 -5 , which predicted possible separation of Al in 2 stages at A/O ratio of 2 .
	manualset3
197538	6	416185	7	NULL	NULL	0	NULL	O : A ratio 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using 0.45 M PC 88 A , extraction isotherm was obtained at an aqueous-to-organic ( A : O ) phase ratio of 1 : 1 -3 and O : A ratio of 1 : 1 -5 , which predicted possible separation of Al in 2 stages at A/O ratio of 2 .
	manualset3
197539	7	416185	7	NULL	NULL	0	NULL	1 : 1 -5	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using 0.45 M PC 88 A , extraction isotherm was obtained at an aqueous-to-organic ( A : O ) phase ratio of 1 : 1 -3 and O : A ratio of 1 : 1 -5 , which predicted possible separation of Al in 2 stages at A/O ratio of 2 .
	manualset3
197540	8	416185	7	NULL	NULL	0	NULL	separation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using 0.45 M PC 88 A , extraction isotherm was obtained at an aqueous-to-organic ( A : O ) phase ratio of 1 : 1 -3 and O : A ratio of 1 : 1 -5 , which predicted possible separation of Al in 2 stages at A/O ratio of 2 .
	manualset3
197541	9	416185	7	NULL	NULL	0	NULL	Al	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using 0.45 M PC 88 A , extraction isotherm was obtained at an aqueous-to-organic ( A : O ) phase ratio of 1 : 1 -3 and O : A ratio of 1 : 1 -5 , which predicted possible separation of Al in 2 stages at A/O ratio of 2 .
	manualset3
197542	10	416185	7	NULL	NULL	0	NULL	2 stages	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using 0.45 M PC 88 A , extraction isotherm was obtained at an aqueous-to-organic ( A : O ) phase ratio of 1 : 1 -3 and O : A ratio of 1 : 1 -5 , which predicted possible separation of Al in 2 stages at A/O ratio of 2 .
	manualset3
197543	11	416185	7	NULL	NULL	0	NULL	A/O ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using 0.45 M PC 88 A , extraction isotherm was obtained at an aqueous-to-organic ( A : O ) phase ratio of 1 : 1 -3 and O : A ratio of 1 : 1 -5 , which predicted possible separation of Al in 2 stages at A/O ratio of 2 .
	manualset3
197544	12	416185	7	NULL	NULL	0	NULL	 2	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using 0.45 M PC 88 A , extraction isotherm was obtained at an aqueous-to-organic ( A : O ) phase ratio of 1 : 1 -3 and O : A ratio of 1 : 1 -5 , which predicted possible separation of Al in 2 stages at A/O ratio of 2 .
	manualset3
197545	1	416186	7	NULL	NULL	0	NULL	12 substrates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using 12 substrates and 6 quaternary inhibitors , the only substantial difference was that the Km for butyrylcholine was 25 times greater for the mutant enzyme , suggesting that butyrylcholine and the organophosphates and carbamates shared a common binding site .
	manualset3
197546	2	416186	7	NULL	NULL	0	NULL	 6 quaternary inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using 12 substrates and 6 quaternary inhibitors , the only substantial difference was that the Km for butyrylcholine was 25 times greater for the mutant enzyme , suggesting that butyrylcholine and the organophosphates and carbamates shared a common binding site .
	manualset3
197547	3	416186	7	NULL	NULL	0	NULL	 substantial difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Using 12 substrates and 6 quaternary inhibitors , the only substantial difference was that the Km for butyrylcholine was 25 times greater for the mutant enzyme , suggesting that butyrylcholine and the organophosphates and carbamates shared a common binding site .
	manualset3
197548	4	416186	7	NULL	NULL	0	NULL	Km	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using 12 substrates and 6 quaternary inhibitors , the only substantial difference was that the Km for butyrylcholine was 25 times greater for the mutant enzyme , suggesting that butyrylcholine and the organophosphates and carbamates shared a common binding site .
	manualset3
197549	5	416186	7	NULL	NULL	0	NULL	 butyrylcholine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using 12 substrates and 6 quaternary inhibitors , the only substantial difference was that the Km for butyrylcholine was 25 times greater for the mutant enzyme , suggesting that butyrylcholine and the organophosphates and carbamates shared a common binding site .
	manualset3
197550	6	416186	7	NULL	NULL	0	NULL	 25 times	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using 12 substrates and 6 quaternary inhibitors , the only substantial difference was that the Km for butyrylcholine was 25 times greater for the mutant enzyme , suggesting that butyrylcholine and the organophosphates and carbamates shared a common binding site .
	manualset3
197551	7	416186	7	NULL	NULL	0	NULL	mutant enzyme	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using 12 substrates and 6 quaternary inhibitors , the only substantial difference was that the Km for butyrylcholine was 25 times greater for the mutant enzyme , suggesting that butyrylcholine and the organophosphates and carbamates shared a common binding site .
	manualset3
197552	8	416186	7	NULL	NULL	0	NULL	butyrylcholine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using 12 substrates and 6 quaternary inhibitors , the only substantial difference was that the Km for butyrylcholine was 25 times greater for the mutant enzyme , suggesting that butyrylcholine and the organophosphates and carbamates shared a common binding site .
	manualset3
197553	9	416186	7	NULL	NULL	0	NULL	 organophosphates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using 12 substrates and 6 quaternary inhibitors , the only substantial difference was that the Km for butyrylcholine was 25 times greater for the mutant enzyme , suggesting that butyrylcholine and the organophosphates and carbamates shared a common binding site .
	manualset3
197554	10	416186	7	NULL	NULL	0	NULL	carbamates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using 12 substrates and 6 quaternary inhibitors , the only substantial difference was that the Km for butyrylcholine was 25 times greater for the mutant enzyme , suggesting that butyrylcholine and the organophosphates and carbamates shared a common binding site .
	manualset3
197555	11	416186	7	NULL	NULL	0	NULL	common binding site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using 12 substrates and 6 quaternary inhibitors , the only substantial difference was that the Km for butyrylcholine was 25 times greater for the mutant enzyme , suggesting that butyrylcholine and the organophosphates and carbamates shared a common binding site .
	manualset3
197556	1	416187	7	NULL	NULL	0	NULL	AHD	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using AHD and tyrosine hydroxylase ( TH ) as immunohistochemical markers , we determined whether differential dissection of the embryonic ( E16 ) ventral mesencephalon ( VM ) into its lateral and medial portions contributed equally to the number of TH cells surviving transplantation , if grafted AHD/TH neurons reinnervate the host striatum according to their normal projection patterns , and examined the functional recovery caused by the implanted cells as assessed by amphetamine-induced rotation in a 6-OHDA-lesioned model of Parkinson 's disease .
	manualset3
197557	2	416187	7	NULL	NULL	0	NULL	tyrosine hydroxylase ( TH ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using AHD and tyrosine hydroxylase ( TH ) as immunohistochemical markers , we determined whether differential dissection of the embryonic ( E16 ) ventral mesencephalon ( VM ) into its lateral and medial portions contributed equally to the number of TH cells surviving transplantation , if grafted AHD/TH neurons reinnervate the host striatum according to their normal projection patterns , and examined the functional recovery caused by the implanted cells as assessed by amphetamine-induced rotation in a 6-OHDA-lesioned model of Parkinson 's disease .
	manualset3
197558	3	416187	7	NULL	NULL	0	NULL	immunohistochemical markers	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using AHD and tyrosine hydroxylase ( TH ) as immunohistochemical markers , we determined whether differential dissection of the embryonic ( E16 ) ventral mesencephalon ( VM ) into its lateral and medial portions contributed equally to the number of TH cells surviving transplantation , if grafted AHD/TH neurons reinnervate the host striatum according to their normal projection patterns , and examined the functional recovery caused by the implanted cells as assessed by amphetamine-induced rotation in a 6-OHDA-lesioned model of Parkinson 's disease .
	manualset3
197559	4	416187	7	NULL	NULL	0	NULL	differential dissection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using AHD and tyrosine hydroxylase ( TH ) as immunohistochemical markers , we determined whether differential dissection of the embryonic ( E16 ) ventral mesencephalon ( VM ) into its lateral and medial portions contributed equally to the number of TH cells surviving transplantation , if grafted AHD/TH neurons reinnervate the host striatum according to their normal projection patterns , and examined the functional recovery caused by the implanted cells as assessed by amphetamine-induced rotation in a 6-OHDA-lesioned model of Parkinson 's disease .
	manualset3
197560	5	416187	7	NULL	NULL	0	NULL	embryonic ( E16 ) ventral mesencephalon ( VM )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Using AHD and tyrosine hydroxylase ( TH ) as immunohistochemical markers , we determined whether differential dissection of the embryonic ( E16 ) ventral mesencephalon ( VM ) into its lateral and medial portions contributed equally to the number of TH cells surviving transplantation , if grafted AHD/TH neurons reinnervate the host striatum according to their normal projection patterns , and examined the functional recovery caused by the implanted cells as assessed by amphetamine-induced rotation in a 6-OHDA-lesioned model of Parkinson 's disease .
	manualset3
197561	6	416187	7	NULL	NULL	0	NULL	lateral and medial portions 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Using AHD and tyrosine hydroxylase ( TH ) as immunohistochemical markers , we determined whether differential dissection of the embryonic ( E16 ) ventral mesencephalon ( VM ) into its lateral and medial portions contributed equally to the number of TH cells surviving transplantation , if grafted AHD/TH neurons reinnervate the host striatum according to their normal projection patterns , and examined the functional recovery caused by the implanted cells as assessed by amphetamine-induced rotation in a 6-OHDA-lesioned model of Parkinson 's disease .
	manualset3
197562	7	416187	7	NULL	NULL	0	NULL	 number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using AHD and tyrosine hydroxylase ( TH ) as immunohistochemical markers , we determined whether differential dissection of the embryonic ( E16 ) ventral mesencephalon ( VM ) into its lateral and medial portions contributed equally to the number of TH cells surviving transplantation , if grafted AHD/TH neurons reinnervate the host striatum according to their normal projection patterns , and examined the functional recovery caused by the implanted cells as assessed by amphetamine-induced rotation in a 6-OHDA-lesioned model of Parkinson 's disease .
	manualset3
197563	8	416187	7	NULL	NULL	0	NULL	TH cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using AHD and tyrosine hydroxylase ( TH ) as immunohistochemical markers , we determined whether differential dissection of the embryonic ( E16 ) ventral mesencephalon ( VM ) into its lateral and medial portions contributed equally to the number of TH cells surviving transplantation , if grafted AHD/TH neurons reinnervate the host striatum according to their normal projection patterns , and examined the functional recovery caused by the implanted cells as assessed by amphetamine-induced rotation in a 6-OHDA-lesioned model of Parkinson 's disease .
	manualset3
197564	9	416187	7	NULL	NULL	0	NULL	transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Using AHD and tyrosine hydroxylase ( TH ) as immunohistochemical markers , we determined whether differential dissection of the embryonic ( E16 ) ventral mesencephalon ( VM ) into its lateral and medial portions contributed equally to the number of TH cells surviving transplantation , if grafted AHD/TH neurons reinnervate the host striatum according to their normal projection patterns , and examined the functional recovery caused by the implanted cells as assessed by amphetamine-induced rotation in a 6-OHDA-lesioned model of Parkinson 's disease .
	manualset3
197565	10	416187	7	NULL	NULL	0	NULL	grafted AHD/TH neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using AHD and tyrosine hydroxylase ( TH ) as immunohistochemical markers , we determined whether differential dissection of the embryonic ( E16 ) ventral mesencephalon ( VM ) into its lateral and medial portions contributed equally to the number of TH cells surviving transplantation , if grafted AHD/TH neurons reinnervate the host striatum according to their normal projection patterns , and examined the functional recovery caused by the implanted cells as assessed by amphetamine-induced rotation in a 6-OHDA-lesioned model of Parkinson 's disease .
	manualset3
197566	11	416187	7	NULL	NULL	0	NULL	host striatum 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Using AHD and tyrosine hydroxylase ( TH ) as immunohistochemical markers , we determined whether differential dissection of the embryonic ( E16 ) ventral mesencephalon ( VM ) into its lateral and medial portions contributed equally to the number of TH cells surviving transplantation , if grafted AHD/TH neurons reinnervate the host striatum according to their normal projection patterns , and examined the functional recovery caused by the implanted cells as assessed by amphetamine-induced rotation in a 6-OHDA-lesioned model of Parkinson 's disease .
	manualset3
197568	12	416187	7	NULL	NULL	0	NULL	normal projection patterns	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using AHD and tyrosine hydroxylase ( TH ) as immunohistochemical markers , we determined whether differential dissection of the embryonic ( E16 ) ventral mesencephalon ( VM ) into its lateral and medial portions contributed equally to the number of TH cells surviving transplantation , if grafted AHD/TH neurons reinnervate the host striatum according to their normal projection patterns , and examined the functional recovery caused by the implanted cells as assessed by amphetamine-induced rotation in a 6-OHDA-lesioned model of Parkinson 's disease .
	manualset3
197569	13	416187	7	NULL	NULL	0	NULL	functional recovery	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using AHD and tyrosine hydroxylase ( TH ) as immunohistochemical markers , we determined whether differential dissection of the embryonic ( E16 ) ventral mesencephalon ( VM ) into its lateral and medial portions contributed equally to the number of TH cells surviving transplantation , if grafted AHD/TH neurons reinnervate the host striatum according to their normal projection patterns , and examined the functional recovery caused by the implanted cells as assessed by amphetamine-induced rotation in a 6-OHDA-lesioned model of Parkinson 's disease .
	manualset3
197570	14	416187	7	NULL	NULL	0	NULL	implanted cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using AHD and tyrosine hydroxylase ( TH ) as immunohistochemical markers , we determined whether differential dissection of the embryonic ( E16 ) ventral mesencephalon ( VM ) into its lateral and medial portions contributed equally to the number of TH cells surviving transplantation , if grafted AHD/TH neurons reinnervate the host striatum according to their normal projection patterns , and examined the functional recovery caused by the implanted cells as assessed by amphetamine-induced rotation in a 6-OHDA-lesioned model of Parkinson 's disease .
	manualset3
197571	15	416187	7	NULL	NULL	0	NULL	amphetamine-induced rotation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using AHD and tyrosine hydroxylase ( TH ) as immunohistochemical markers , we determined whether differential dissection of the embryonic ( E16 ) ventral mesencephalon ( VM ) into its lateral and medial portions contributed equally to the number of TH cells surviving transplantation , if grafted AHD/TH neurons reinnervate the host striatum according to their normal projection patterns , and examined the functional recovery caused by the implanted cells as assessed by amphetamine-induced rotation in a 6-OHDA-lesioned model of Parkinson 's disease .
	manualset3
197572	16	416187	7	NULL	NULL	0	NULL	 6-OHDA-lesioned model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Using AHD and tyrosine hydroxylase ( TH ) as immunohistochemical markers , we determined whether differential dissection of the embryonic ( E16 ) ventral mesencephalon ( VM ) into its lateral and medial portions contributed equally to the number of TH cells surviving transplantation , if grafted AHD/TH neurons reinnervate the host striatum according to their normal projection patterns , and examined the functional recovery caused by the implanted cells as assessed by amphetamine-induced rotation in a 6-OHDA-lesioned model of Parkinson 's disease .
	manualset3
197573	17	416187	7	NULL	NULL	0	NULL	Parkinson 's disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Using AHD and tyrosine hydroxylase ( TH ) as immunohistochemical markers , we determined whether differential dissection of the embryonic ( E16 ) ventral mesencephalon ( VM ) into its lateral and medial portions contributed equally to the number of TH cells surviving transplantation , if grafted AHD/TH neurons reinnervate the host striatum according to their normal projection patterns , and examined the functional recovery caused by the implanted cells as assessed by amphetamine-induced rotation in a 6-OHDA-lesioned model of Parkinson 's disease .
	manualset3
197574	1	416188	7	NULL	NULL	0	NULL	Benner 's philosophy	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Benner 's philosophy that identifies the importance of acknowledging one 's accomplishments and being acknowledged by others , the authors present the design implementation , and evaluation of a Professional Nurse Advancement Program ( PNAP ) .
	manualset3
197575	2	416188	7	NULL	NULL	0	NULL	accomplishments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Benner 's philosophy that identifies the importance of acknowledging one 's accomplishments and being acknowledged by others , the authors present the design implementation , and evaluation of a Professional Nurse Advancement Program ( PNAP ) .
	manualset3
197576	3	416188	7	NULL	NULL	0	NULL	 authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Benner 's philosophy that identifies the importance of acknowledging one 's accomplishments and being acknowledged by others , the authors present the design implementation , and evaluation of a Professional Nurse Advancement Program ( PNAP ) .
	manualset3
197577	4	416188	7	NULL	NULL	0	NULL	design implementation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Benner 's philosophy that identifies the importance of acknowledging one 's accomplishments and being acknowledged by others , the authors present the design implementation , and evaluation of a Professional Nurse Advancement Program ( PNAP ) .
	manualset3
197578	5	416188	7	NULL	NULL	0	NULL	evaluation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Benner 's philosophy that identifies the importance of acknowledging one 's accomplishments and being acknowledged by others , the authors present the design implementation , and evaluation of a Professional Nurse Advancement Program ( PNAP ) .
	manualset3
197579	6	416188	7	NULL	NULL	0	NULL	Professional Nurse Advancement Program ( PNAP )	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Benner 's philosophy that identifies the importance of acknowledging one 's accomplishments and being acknowledged by others , the authors present the design implementation , and evaluation of a Professional Nurse Advancement Program ( PNAP ) .
	manualset3
197580	1	416189	7	NULL	NULL	0	NULL	CMR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using CMR , LV end-diastolic volume ( EDV ) , mass ( LVM ) , ejection fraction , ( cc ) and myocardial delayed enhancement ( MDE ) were determined in DMD patients and normal control subjects .
	manualset3
197581	2	416189	7	NULL	NULL	0	NULL	LV end-diastolic volume ( EDV )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using CMR , LV end-diastolic volume ( EDV ) , mass ( LVM ) , ejection fraction , ( cc ) and myocardial delayed enhancement ( MDE ) were determined in DMD patients and normal control subjects .
	manualset3
197582	3	416189	7	NULL	NULL	0	NULL	mass ( LVM )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using CMR , LV end-diastolic volume ( EDV ) , mass ( LVM ) , ejection fraction , ( cc ) and myocardial delayed enhancement ( MDE ) were determined in DMD patients and normal control subjects .
	manualset3
197583	4	416189	7	NULL	NULL	0	NULL	ejection fraction ( cc )	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using CMR , LV end-diastolic volume ( EDV ) , mass ( LVM ) , ejection fraction , ( cc ) and myocardial delayed enhancement ( MDE ) were determined in DMD patients and normal control subjects .
	manualset3
197584	5	416189	7	NULL	NULL	0	NULL	myocardial delayed enhancement ( MDE )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using CMR , LV end-diastolic volume ( EDV ) , mass ( LVM ) , ejection fraction , ( cc ) and myocardial delayed enhancement ( MDE ) were determined in DMD patients and normal control subjects .
	manualset3
197585	6	416189	7	NULL	NULL	0	NULL	DMD patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using CMR , LV end-diastolic volume ( EDV ) , mass ( LVM ) , ejection fraction , ( cc ) and myocardial delayed enhancement ( MDE ) were determined in DMD patients and normal control subjects .
	manualset3
197586	7	416189	7	NULL	NULL	0	NULL	normal control subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using CMR , LV end-diastolic volume ( EDV ) , mass ( LVM ) , ejection fraction , ( cc ) and myocardial delayed enhancement ( MDE ) were determined in DMD patients and normal control subjects .
	manualset3
197587	1	416190	7	NULL	NULL	0	NULL	GLUT1-transfected CHO cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using GLUT1-transfected CHO cells , we demonstrated that increased expression of GLUT1 was paralleled by a corresponding increase in hexose transport but that there were no changes in nicotinamide transport .
	manualset3
197588	2	416190	7	NULL	NULL	0	NULL	increased expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using GLUT1-transfected CHO cells , we demonstrated that increased expression of GLUT1 was paralleled by a corresponding increase in hexose transport but that there were no changes in nicotinamide transport .
	manualset3
197589	3	416190	7	NULL	NULL	0	NULL	GLUT1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using GLUT1-transfected CHO cells , we demonstrated that increased expression of GLUT1 was paralleled by a corresponding increase in hexose transport but that there were no changes in nicotinamide transport .
	manualset3
197590	4	416190	7	NULL	NULL	0	NULL	hexose transport	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using GLUT1-transfected CHO cells , we demonstrated that increased expression of GLUT1 was paralleled by a corresponding increase in hexose transport but that there were no changes in nicotinamide transport .
	manualset3
197591	5	416190	7	NULL	NULL	0	NULL	no changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using GLUT1-transfected CHO cells , we demonstrated that increased expression of GLUT1 was paralleled by a corresponding increase in hexose transport but that there were no changes in nicotinamide transport .
	manualset3
197592	6	416190	7	NULL	NULL	0	NULL	nicotinamide transport	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using GLUT1-transfected CHO cells , we demonstrated that increased expression of GLUT1 was paralleled by a corresponding increase in hexose transport but that there were no changes in nicotinamide transport .
	manualset3
197593	1	416191	7	NULL	NULL	0	NULL	Generalized Estimating Equations analyses	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Generalized Estimating Equations analyses , the IAT effect was positively associated with pre-task craving ratings assessed on the Questionnaire of Smoking Urges-Brief but was not associated with a physiological measure of automatic affective responses ( startles while viewing smoking versus neutral pictures ) .
	manualset3
197594	2	416191	7	NULL	NULL	0	NULL	 IAT effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Generalized Estimating Equations analyses , the IAT effect was positively associated with pre-task craving ratings assessed on the Questionnaire of Smoking Urges-Brief but was not associated with a physiological measure of automatic affective responses ( startles while viewing smoking versus neutral pictures ) .
	manualset3
197595	3	416191	7	NULL	NULL	0	NULL	pre-task craving ratings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Generalized Estimating Equations analyses , the IAT effect was positively associated with pre-task craving ratings assessed on the Questionnaire of Smoking Urges-Brief but was not associated with a physiological measure of automatic affective responses ( startles while viewing smoking versus neutral pictures ) .
	manualset3
197596	4	416191	7	NULL	NULL	0	NULL	Questionnaire	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Generalized Estimating Equations analyses , the IAT effect was positively associated with pre-task craving ratings assessed on the Questionnaire of Smoking Urges-Brief but was not associated with a physiological measure of automatic affective responses ( startles while viewing smoking versus neutral pictures ) .
	manualset3
197597	5	416191	7	NULL	NULL	0	NULL	Smoking Urges-Brief 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Generalized Estimating Equations analyses , the IAT effect was positively associated with pre-task craving ratings assessed on the Questionnaire of Smoking Urges-Brief but was not associated with a physiological measure of automatic affective responses ( startles while viewing smoking versus neutral pictures ) .
	manualset3
197598	6	416191	7	NULL	NULL	0	NULL	physiological measure 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Generalized Estimating Equations analyses , the IAT effect was positively associated with pre-task craving ratings assessed on the Questionnaire of Smoking Urges-Brief but was not associated with a physiological measure of automatic affective responses ( startles while viewing smoking versus neutral pictures ) .
	manualset3
197599	7	416191	7	NULL	NULL	0	NULL	 automatic affective responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Generalized Estimating Equations analyses , the IAT effect was positively associated with pre-task craving ratings assessed on the Questionnaire of Smoking Urges-Brief but was not associated with a physiological measure of automatic affective responses ( startles while viewing smoking versus neutral pictures ) .
	manualset3
197600	8	416191	7	NULL	NULL	0	NULL	smoking	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Generalized Estimating Equations analyses , the IAT effect was positively associated with pre-task craving ratings assessed on the Questionnaire of Smoking Urges-Brief but was not associated with a physiological measure of automatic affective responses ( startles while viewing smoking versus neutral pictures ) .
	manualset3
197601	9	416191	7	NULL	NULL	0	NULL	 neutral pictures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Generalized Estimating Equations analyses , the IAT effect was positively associated with pre-task craving ratings assessed on the Questionnaire of Smoking Urges-Brief but was not associated with a physiological measure of automatic affective responses ( startles while viewing smoking versus neutral pictures ) .
	manualset3
197602	1	416192	7	NULL	NULL	0	NULL	ICD9-CM discharge codes	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Using ICD9-CM discharge codes , we identified patients with an associated complication .
	manualset3
197603	2	416192	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using ICD9-CM discharge codes , we identified patients with an associated complication .
	manualset3
197604	3	416192	7	NULL	NULL	0	NULL	associated complication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using ICD9-CM discharge codes , we identified patients with an associated complication .
	manualset3
197605	1	416193	7	NULL	NULL	0	NULL	IgG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using IgG from these sera , we showed that the DNA protected from degradation remained bound to IgG during digestion and was 35-45 base pairs in size .
	manualset3
197606	2	416193	7	NULL	NULL	0	NULL	sera	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using IgG from these sera , we showed that the DNA protected from degradation remained bound to IgG during digestion and was 35-45 base pairs in size .
	manualset3
197607	3	416193	7	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using IgG from these sera , we showed that the DNA protected from degradation remained bound to IgG during digestion and was 35-45 base pairs in size .
	manualset3
197608	4	416193	7	NULL	NULL	0	NULL	degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using IgG from these sera , we showed that the DNA protected from degradation remained bound to IgG during digestion and was 35-45 base pairs in size .
	manualset3
197609	5	416193	7	NULL	NULL	0	NULL	IgG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using IgG from these sera , we showed that the DNA protected from degradation remained bound to IgG during digestion and was 35-45 base pairs in size .
	manualset3
197610	6	416193	7	NULL	NULL	0	NULL	digestion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using IgG from these sera , we showed that the DNA protected from degradation remained bound to IgG during digestion and was 35-45 base pairs in size .
	manualset3
197611	7	416193	7	NULL	NULL	0	NULL	35-45 base pairs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using IgG from these sera , we showed that the DNA protected from degradation remained bound to IgG during digestion and was 35-45 base pairs in size .
	manualset3
197612	8	416193	7	NULL	NULL	0	NULL	size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using IgG from these sera , we showed that the DNA protected from degradation remained bound to IgG during digestion and was 35-45 base pairs in size .
	manualset3
197613	1	416194	7	NULL	NULL	0	NULL	transportation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After transportation at 0 degree C from the operation room , the hearts were quickly rewarmed to 37 degrees C. Serial transmural biopsy specimens were taken during normothermic ischemia for determination of purine catabolites .
	manualset3
197614	2	416194	7	NULL	NULL	0	NULL	 0 degree C	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After transportation at 0 degree C from the operation room , the hearts were quickly rewarmed to 37 degrees C. Serial transmural biopsy specimens were taken during normothermic ischemia for determination of purine catabolites .
	manualset3
197615	3	416194	7	NULL	NULL	0	NULL	operation room	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	After transportation at 0 degree C from the operation room , the hearts were quickly rewarmed to 37 degrees C. Serial transmural biopsy specimens were taken during normothermic ischemia for determination of purine catabolites .
	manualset3
197616	4	416194	7	NULL	NULL	0	NULL	 hearts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After transportation at 0 degree C from the operation room , the hearts were quickly rewarmed to 37 degrees C. Serial transmural biopsy specimens were taken during normothermic ischemia for determination of purine catabolites .
	manualset3
197617	5	416194	7	NULL	NULL	0	NULL	37 degrees C.	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After transportation at 0 degree C from the operation room , the hearts were quickly rewarmed to 37 degrees C. Serial transmural biopsy specimens were taken during normothermic ischemia for determination of purine catabolites .
	manualset3
197618	6	416194	7	NULL	NULL	0	NULL	Serial transmural biopsy specimens	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	After transportation at 0 degree C from the operation room , the hearts were quickly rewarmed to 37 degrees C. Serial transmural biopsy specimens were taken during normothermic ischemia for determination of purine catabolites .
	manualset3
197619	7	416194	7	NULL	NULL	0	NULL	normothermic ischemia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	After transportation at 0 degree C from the operation room , the hearts were quickly rewarmed to 37 degrees C. Serial transmural biopsy specimens were taken during normothermic ischemia for determination of purine catabolites .
	manualset3
197620	8	416194	7	NULL	NULL	0	NULL	 determination	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After transportation at 0 degree C from the operation room , the hearts were quickly rewarmed to 37 degrees C. Serial transmural biopsy specimens were taken during normothermic ischemia for determination of purine catabolites .
	manualset3
197621	9	416194	7	NULL	NULL	0	NULL	 purine catabolites	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After transportation at 0 degree C from the operation room , the hearts were quickly rewarmed to 37 degrees C. Serial transmural biopsy specimens were taken during normothermic ischemia for determination of purine catabolites .
	manualset3
197622	1	416195	7	NULL	NULL	0	NULL	Mann-Whitney 's U	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Mann-Whitney 's U the mean of anti-GAD65 in diabetic type 1 and 2 patients was p = 0.022 ; between DM1 and their siblings and between DM2 and their siblings there was no statistical significance .
	manualset3
197623	2	416195	7	NULL	NULL	0	NULL	mean	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Mann-Whitney 's U the mean of anti-GAD65 in diabetic type 1 and 2 patients was p = 0.022 ; between DM1 and their siblings and between DM2 and their siblings there was no statistical significance .
	manualset3
197624	3	416195	7	NULL	NULL	0	NULL	anti-GAD65 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Mann-Whitney 's U the mean of anti-GAD65 in diabetic type 1 and 2 patients was p = 0.022 ; between DM1 and their siblings and between DM2 and their siblings there was no statistical significance .
	manualset3
197625	4	416195	7	NULL	NULL	0	NULL	diabetic type 1	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Mann-Whitney 's U the mean of anti-GAD65 in diabetic type 1 and 2 patients was p = 0.022 ; between DM1 and their siblings and between DM2 and their siblings there was no statistical significance .
	manualset3
197626	5	416195	7	NULL	NULL	0	NULL	diabetic type 2	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Mann-Whitney 's U the mean of anti-GAD65 in diabetic type 1 and 2 patients was p = 0.022 ; between DM1 and their siblings and between DM2 and their siblings there was no statistical significance .
	manualset3
197627	6	416195	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Mann-Whitney 's U the mean of anti-GAD65 in diabetic type 1 and 2 patients was p = 0.022 ; between DM1 and their siblings and between DM2 and their siblings there was no statistical significance .
	manualset3
197628	7	416195	7	NULL	NULL	0	NULL	p = 0.022	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Mann-Whitney 's U the mean of anti-GAD65 in diabetic type 1 and 2 patients was p = 0.022 ; between DM1 and their siblings and between DM2 and their siblings there was no statistical significance .
	manualset3
197629	8	416195	7	NULL	NULL	0	NULL	DM1	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Mann-Whitney 's U the mean of anti-GAD65 in diabetic type 1 and 2 patients was p = 0.022 ; between DM1 and their siblings and between DM2 and their siblings there was no statistical significance .
	manualset3
197630	9	416195	7	NULL	NULL	0	NULL	 siblings	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Mann-Whitney 's U the mean of anti-GAD65 in diabetic type 1 and 2 patients was p = 0.022 ; between DM1 and their siblings and between DM2 and their siblings there was no statistical significance .
	manualset3
197631	10	416195	7	NULL	NULL	0	NULL	DM2	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Mann-Whitney 's U the mean of anti-GAD65 in diabetic type 1 and 2 patients was p = 0.022 ; between DM1 and their siblings and between DM2 and their siblings there was no statistical significance .
	manualset3
197632	11	416195	7	NULL	NULL	0	NULL	siblings	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Mann-Whitney 's U the mean of anti-GAD65 in diabetic type 1 and 2 patients was p = 0.022 ; between DM1 and their siblings and between DM2 and their siblings there was no statistical significance .
	manualset3
197633	12	416195	7	NULL	NULL	0	NULL	statistical significance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Mann-Whitney 's U the mean of anti-GAD65 in diabetic type 1 and 2 patients was p = 0.022 ; between DM1 and their siblings and between DM2 and their siblings there was no statistical significance .
	manualset3
197634	1	416196	7	NULL	NULL	0	NULL	OLS regression models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Using OLS regression models , our findings suggest body composition is not associated with cognitive functioning in adults ages 60-69 ; however , for adults aged 70 and over , sarcopenia and obesity , either independently or concurrently , were associated with worse cognitive functioning relative to non-sarcopenic non-obese older adults .
	manualset3
197635	2	416196	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using OLS regression models , our findings suggest body composition is not associated with cognitive functioning in adults ages 60-69 ; however , for adults aged 70 and over , sarcopenia and obesity , either independently or concurrently , were associated with worse cognitive functioning relative to non-sarcopenic non-obese older adults .
	manualset3
197636	3	416196	7	NULL	NULL	0	NULL	body composition	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using OLS regression models , our findings suggest body composition is not associated with cognitive functioning in adults ages 60-69 ; however , for adults aged 70 and over , sarcopenia and obesity , either independently or concurrently , were associated with worse cognitive functioning relative to non-sarcopenic non-obese older adults .
	manualset3
197637	4	416196	7	NULL	NULL	0	NULL	cognitive functioning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using OLS regression models , our findings suggest body composition is not associated with cognitive functioning in adults ages 60-69 ; however , for adults aged 70 and over , sarcopenia and obesity , either independently or concurrently , were associated with worse cognitive functioning relative to non-sarcopenic non-obese older adults .
	manualset3
197638	5	416196	7	NULL	NULL	0	NULL	adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using OLS regression models , our findings suggest body composition is not associated with cognitive functioning in adults ages 60-69 ; however , for adults aged 70 and over , sarcopenia and obesity , either independently or concurrently , were associated with worse cognitive functioning relative to non-sarcopenic non-obese older adults .
	manualset3
197639	6	416196	7	NULL	NULL	0	NULL	ages 60-69 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Using OLS regression models , our findings suggest body composition is not associated with cognitive functioning in adults ages 60-69 ; however , for adults aged 70 and over , sarcopenia and obesity , either independently or concurrently , were associated with worse cognitive functioning relative to non-sarcopenic non-obese older adults .
	manualset3
197640	7	416196	7	NULL	NULL	0	NULL	adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using OLS regression models , our findings suggest body composition is not associated with cognitive functioning in adults ages 60-69 ; however , for adults aged 70 and over , sarcopenia and obesity , either independently or concurrently , were associated with worse cognitive functioning relative to non-sarcopenic non-obese older adults .
	manualset3
197641	8	416196	7	NULL	NULL	0	NULL	aged 70	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Using OLS regression models , our findings suggest body composition is not associated with cognitive functioning in adults ages 60-69 ; however , for adults aged 70 and over , sarcopenia and obesity , either independently or concurrently , were associated with worse cognitive functioning relative to non-sarcopenic non-obese older adults .
	manualset3
197642	9	416196	7	NULL	NULL	0	NULL	sarcopenia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Using OLS regression models , our findings suggest body composition is not associated with cognitive functioning in adults ages 60-69 ; however , for adults aged 70 and over , sarcopenia and obesity , either independently or concurrently , were associated with worse cognitive functioning relative to non-sarcopenic non-obese older adults .
	manualset3
197643	10	416196	7	NULL	NULL	0	NULL	obesity 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Using OLS regression models , our findings suggest body composition is not associated with cognitive functioning in adults ages 60-69 ; however , for adults aged 70 and over , sarcopenia and obesity , either independently or concurrently , were associated with worse cognitive functioning relative to non-sarcopenic non-obese older adults .
	manualset3
197644	11	416196	7	NULL	NULL	0	NULL	cognitive functioning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using OLS regression models , our findings suggest body composition is not associated with cognitive functioning in adults ages 60-69 ; however , for adults aged 70 and over , sarcopenia and obesity , either independently or concurrently , were associated with worse cognitive functioning relative to non-sarcopenic non-obese older adults .
	manualset3
197645	12	416196	7	NULL	NULL	0	NULL	non-sarcopenic non-obese older adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using OLS regression models , our findings suggest body composition is not associated with cognitive functioning in adults ages 60-69 ; however , for adults aged 70 and over , sarcopenia and obesity , either independently or concurrently , were associated with worse cognitive functioning relative to non-sarcopenic non-obese older adults .
	manualset3
197646	1	416197	7	NULL	NULL	0	NULL	Osh4p/Kes1p	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Osh4p/Kes1p as a representative ORP , we show that ORPs have at least two membrane-binding surfaces ; one near the mouth of the sterol-binding pocket and a distal site that can bind a second membrane .
	manualset3
197647	2	416197	7	NULL	NULL	0	NULL	ORP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Osh4p/Kes1p as a representative ORP , we show that ORPs have at least two membrane-binding surfaces ; one near the mouth of the sterol-binding pocket and a distal site that can bind a second membrane .
	manualset3
197648	3	416197	7	NULL	NULL	0	NULL	ORPs	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Osh4p/Kes1p as a representative ORP , we show that ORPs have at least two membrane-binding surfaces ; one near the mouth of the sterol-binding pocket and a distal site that can bind a second membrane .
	manualset3
197649	4	416197	7	NULL	NULL	0	NULL	 two membrane-binding surfaces	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Osh4p/Kes1p as a representative ORP , we show that ORPs have at least two membrane-binding surfaces ; one near the mouth of the sterol-binding pocket and a distal site that can bind a second membrane .
	manualset3
197650	5	416197	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Osh4p/Kes1p as a representative ORP , we show that ORPs have at least two membrane-binding surfaces ; one near the mouth of the sterol-binding pocket and a distal site that can bind a second membrane .
	manualset3
197651	6	416197	7	NULL	NULL	0	NULL	mouth of the sterol-binding pocket	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Osh4p/Kes1p as a representative ORP , we show that ORPs have at least two membrane-binding surfaces ; one near the mouth of the sterol-binding pocket and a distal site that can bind a second membrane .
	manualset3
197652	7	416197	7	NULL	NULL	0	NULL	distal site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Osh4p/Kes1p as a representative ORP , we show that ORPs have at least two membrane-binding surfaces ; one near the mouth of the sterol-binding pocket and a distal site that can bind a second membrane .
	manualset3
197653	8	416197	7	NULL	NULL	0	NULL	second membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Using Osh4p/Kes1p as a representative ORP , we show that ORPs have at least two membrane-binding surfaces ; one near the mouth of the sterol-binding pocket and a distal site that can bind a second membrane .
	manualset3
197654	1	416198	7	NULL	NULL	0	NULL	 PFGE	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using PFGE , Salmonella isolates obtained from irrigation water and equipment were determined to be different from cantaloupe isolates ; however , DNA fingerprinting did not conclusively define relationships between contamination sources .
	manualset3
197655	2	416198	7	NULL	NULL	0	NULL	Salmonella isolates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Using PFGE , Salmonella isolates obtained from irrigation water and equipment were determined to be different from cantaloupe isolates ; however , DNA fingerprinting did not conclusively define relationships between contamination sources .
	manualset3
197656	3	416198	7	NULL	NULL	0	NULL	 irrigation water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using PFGE , Salmonella isolates obtained from irrigation water and equipment were determined to be different from cantaloupe isolates ; however , DNA fingerprinting did not conclusively define relationships between contamination sources .
	manualset3
197657	4	416198	7	NULL	NULL	0	NULL	equipment	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Using PFGE , Salmonella isolates obtained from irrigation water and equipment were determined to be different from cantaloupe isolates ; however , DNA fingerprinting did not conclusively define relationships between contamination sources .
	manualset3
197658	5	416198	7	NULL	NULL	0	NULL	cantaloupe isolates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Using PFGE , Salmonella isolates obtained from irrigation water and equipment were determined to be different from cantaloupe isolates ; however , DNA fingerprinting did not conclusively define relationships between contamination sources .
	manualset3
197659	6	416198	7	NULL	NULL	0	NULL	DNA fingerprinting	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using PFGE , Salmonella isolates obtained from irrigation water and equipment were determined to be different from cantaloupe isolates ; however , DNA fingerprinting did not conclusively define relationships between contamination sources .
	manualset3
197660	7	416198	7	NULL	NULL	0	NULL	relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Using PFGE , Salmonella isolates obtained from irrigation water and equipment were determined to be different from cantaloupe isolates ; however , DNA fingerprinting did not conclusively define relationships between contamination sources .
	manualset3
197661	8	416198	7	NULL	NULL	0	NULL	contamination sources	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using PFGE , Salmonella isolates obtained from irrigation water and equipment were determined to be different from cantaloupe isolates ; however , DNA fingerprinting did not conclusively define relationships between contamination sources .
	manualset3
197662	1	416199	7	NULL	NULL	0	NULL	RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using RNA allowed a definition of the left ventricular ejection fraction ( LVEF ) , and then calculation of the left ventricular end-diastolic volume ( LVEDV ) , both before and after PEEP .
	manualset3
197663	2	416199	7	NULL	NULL	0	NULL	definition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using RNA allowed a definition of the left ventricular ejection fraction ( LVEF ) , and then calculation of the left ventricular end-diastolic volume ( LVEDV ) , both before and after PEEP .
	manualset3
197664	3	416199	7	NULL	NULL	0	NULL	left ventricular ejection fraction ( LVEF )	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using RNA allowed a definition of the left ventricular ejection fraction ( LVEF ) , and then calculation of the left ventricular end-diastolic volume ( LVEDV ) , both before and after PEEP .
	manualset3
197665	4	416199	7	NULL	NULL	0	NULL	 calculation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using RNA allowed a definition of the left ventricular ejection fraction ( LVEF ) , and then calculation of the left ventricular end-diastolic volume ( LVEDV ) , both before and after PEEP .
	manualset3
197666	5	416199	7	NULL	NULL	0	NULL	 left ventricular end-diastolic volume ( LVEDV )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using RNA allowed a definition of the left ventricular ejection fraction ( LVEF ) , and then calculation of the left ventricular end-diastolic volume ( LVEDV ) , both before and after PEEP .
	manualset3
197667	6	416199	7	NULL	NULL	0	NULL	PEEP	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using RNA allowed a definition of the left ventricular ejection fraction ( LVEF ) , and then calculation of the left ventricular end-diastolic volume ( LVEDV ) , both before and after PEEP .
	manualset3
197668	1	416200	7	NULL	NULL	0	NULL	RT-PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using RT-PCR we demonstrate that normal human bronchial epithelial ( NHBE ) cells upon ligation of K1T with specific Abs caused upregulation of pro-fibrotic growth factors .
	manualset3
197669	2	416200	7	NULL	NULL	0	NULL	normal human bronchial epithelial ( NHBE ) cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using RT-PCR we demonstrate that normal human bronchial epithelial ( NHBE ) cells upon ligation of K1T with specific Abs caused upregulation of pro-fibrotic growth factors .
	manualset3
197670	3	416200	7	NULL	NULL	0	NULL	ligation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using RT-PCR we demonstrate that normal human bronchial epithelial ( NHBE ) cells upon ligation of K1T with specific Abs caused upregulation of pro-fibrotic growth factors .
	manualset3
197671	4	416200	7	NULL	NULL	0	NULL	K1T	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using RT-PCR we demonstrate that normal human bronchial epithelial ( NHBE ) cells upon ligation of K1T with specific Abs caused upregulation of pro-fibrotic growth factors .
	manualset3
197672	5	416200	7	NULL	NULL	0	NULL	specific Abs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using RT-PCR we demonstrate that normal human bronchial epithelial ( NHBE ) cells upon ligation of K1T with specific Abs caused upregulation of pro-fibrotic growth factors .
	manualset3
197673	6	416200	7	NULL	NULL	0	NULL	upregulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using RT-PCR we demonstrate that normal human bronchial epithelial ( NHBE ) cells upon ligation of K1T with specific Abs caused upregulation of pro-fibrotic growth factors .
	manualset3
197674	7	416200	7	NULL	NULL	NULL	NULL	pro-fibrotic growth factors	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using RT-PCR we demonstrate that normal human bronchial epithelial ( NHBE ) cells upon ligation of K1T with specific Abs caused upregulation of pro-fibrotic growth factors .
	manualset3
197675	1	416201	7	NULL	NULL	0	NULL	Huntington disease cell model	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a Huntington disease cell model , we have demonstrated that feeble interaction of HIP1 with mutant huntingtin protein resulted in increased nuclear accumulation of HIPPI and HIP1 , leading to higher occupancy of HIPPI at the REST promoter , triggering its transcriptional activation and consequent repression of REST target genes .
	manualset3
197676	2	416201	7	NULL	NULL	0	NULL	feeble interaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a Huntington disease cell model , we have demonstrated that feeble interaction of HIP1 with mutant huntingtin protein resulted in increased nuclear accumulation of HIPPI and HIP1 , leading to higher occupancy of HIPPI at the REST promoter , triggering its transcriptional activation and consequent repression of REST target genes .
	manualset3
197677	3	416201	7	NULL	NULL	0	NULL	 HIP1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a Huntington disease cell model , we have demonstrated that feeble interaction of HIP1 with mutant huntingtin protein resulted in increased nuclear accumulation of HIPPI and HIP1 , leading to higher occupancy of HIPPI at the REST promoter , triggering its transcriptional activation and consequent repression of REST target genes .
	manualset3
197678	4	416201	7	NULL	NULL	0	NULL	mutant huntingtin protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a Huntington disease cell model , we have demonstrated that feeble interaction of HIP1 with mutant huntingtin protein resulted in increased nuclear accumulation of HIPPI and HIP1 , leading to higher occupancy of HIPPI at the REST promoter , triggering its transcriptional activation and consequent repression of REST target genes .
	manualset3
197679	5	416201	7	NULL	NULL	0	NULL	increased nuclear accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a Huntington disease cell model , we have demonstrated that feeble interaction of HIP1 with mutant huntingtin protein resulted in increased nuclear accumulation of HIPPI and HIP1 , leading to higher occupancy of HIPPI at the REST promoter , triggering its transcriptional activation and consequent repression of REST target genes .
	manualset3
197680	6	416201	7	NULL	NULL	0	NULL	HIPPI	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a Huntington disease cell model , we have demonstrated that feeble interaction of HIP1 with mutant huntingtin protein resulted in increased nuclear accumulation of HIPPI and HIP1 , leading to higher occupancy of HIPPI at the REST promoter , triggering its transcriptional activation and consequent repression of REST target genes .
	manualset3
197681	7	416201	7	NULL	NULL	0	NULL	 HIP1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a Huntington disease cell model , we have demonstrated that feeble interaction of HIP1 with mutant huntingtin protein resulted in increased nuclear accumulation of HIPPI and HIP1 , leading to higher occupancy of HIPPI at the REST promoter , triggering its transcriptional activation and consequent repression of REST target genes .
	manualset3
197682	8	416201	7	NULL	NULL	0	NULL	 higher occupancy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a Huntington disease cell model , we have demonstrated that feeble interaction of HIP1 with mutant huntingtin protein resulted in increased nuclear accumulation of HIPPI and HIP1 , leading to higher occupancy of HIPPI at the REST promoter , triggering its transcriptional activation and consequent repression of REST target genes .
	manualset3
197683	9	416201	7	NULL	NULL	0	NULL	HIPPI	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a Huntington disease cell model , we have demonstrated that feeble interaction of HIP1 with mutant huntingtin protein resulted in increased nuclear accumulation of HIPPI and HIP1 , leading to higher occupancy of HIPPI at the REST promoter , triggering its transcriptional activation and consequent repression of REST target genes .
	manualset3
197684	10	416201	7	NULL	NULL	0	NULL	REST promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a Huntington disease cell model , we have demonstrated that feeble interaction of HIP1 with mutant huntingtin protein resulted in increased nuclear accumulation of HIPPI and HIP1 , leading to higher occupancy of HIPPI at the REST promoter , triggering its transcriptional activation and consequent repression of REST target genes .
	manualset3
197685	11	416201	7	NULL	NULL	0	NULL	transcriptional activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a Huntington disease cell model , we have demonstrated that feeble interaction of HIP1 with mutant huntingtin protein resulted in increased nuclear accumulation of HIPPI and HIP1 , leading to higher occupancy of HIPPI at the REST promoter , triggering its transcriptional activation and consequent repression of REST target genes .
	manualset3
197686	12	416201	7	NULL	NULL	0	NULL	consequent repression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a Huntington disease cell model , we have demonstrated that feeble interaction of HIP1 with mutant huntingtin protein resulted in increased nuclear accumulation of HIPPI and HIP1 , leading to higher occupancy of HIPPI at the REST promoter , triggering its transcriptional activation and consequent repression of REST target genes .
	manualset3
197687	13	416201	7	NULL	NULL	0	NULL	REST target genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a Huntington disease cell model , we have demonstrated that feeble interaction of HIP1 with mutant huntingtin protein resulted in increased nuclear accumulation of HIPPI and HIP1 , leading to higher occupancy of HIPPI at the REST promoter , triggering its transcriptional activation and consequent repression of REST target genes .
	manualset3
197688	1	416202	7	NULL	NULL	0	NULL	competitive reverse transcription-polymerase chain reaction method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a competitive reverse transcription-polymerase chain reaction method , we demonstrated that M2 receptor gene expression was decreased by more that an order of magnitude both by virus infection and by treatment with IFN .
	manualset3
197689	2	416202	7	NULL	NULL	0	NULL	M2 receptor gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a competitive reverse transcription-polymerase chain reaction method , we demonstrated that M2 receptor gene expression was decreased by more that an order of magnitude both by virus infection and by treatment with IFN .
	manualset3
197690	3	416202	7	NULL	NULL	0	NULL	order of magnitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a competitive reverse transcription-polymerase chain reaction method , we demonstrated that M2 receptor gene expression was decreased by more that an order of magnitude both by virus infection and by treatment with IFN .
	manualset3
197691	4	416202	7	NULL	NULL	0	NULL	virus infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a competitive reverse transcription-polymerase chain reaction method , we demonstrated that M2 receptor gene expression was decreased by more that an order of magnitude both by virus infection and by treatment with IFN .
	manualset3
197692	5	416202	7	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a competitive reverse transcription-polymerase chain reaction method , we demonstrated that M2 receptor gene expression was decreased by more that an order of magnitude both by virus infection and by treatment with IFN .
	manualset3
197693	6	416202	7	NULL	NULL	0	NULL	IFN	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a competitive reverse transcription-polymerase chain reaction method , we demonstrated that M2 receptor gene expression was decreased by more that an order of magnitude both by virus infection and by treatment with IFN .
	manualset3
197694	1	416203	7	NULL	NULL	0	NULL	composite model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a composite model of the glucose homeostasis system , consisting of seven interconnected submodels , we enumerate the possible behaviors of the model in response to variation of liver insulin sensitivity and dietary glucose variability .
	manualset3
197695	2	416203	7	NULL	NULL	0	NULL	glucose homeostasis system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a composite model of the glucose homeostasis system , consisting of seven interconnected submodels , we enumerate the possible behaviors of the model in response to variation of liver insulin sensitivity and dietary glucose variability .
	manualset3
197696	3	416203	7	NULL	NULL	0	NULL	seven interconnected submodels	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a composite model of the glucose homeostasis system , consisting of seven interconnected submodels , we enumerate the possible behaviors of the model in response to variation of liver insulin sensitivity and dietary glucose variability .
	manualset3
197697	4	416203	7	NULL	NULL	0	NULL	 behaviors 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a composite model of the glucose homeostasis system , consisting of seven interconnected submodels , we enumerate the possible behaviors of the model in response to variation of liver insulin sensitivity and dietary glucose variability .
	manualset3
197698	5	416203	7	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a composite model of the glucose homeostasis system , consisting of seven interconnected submodels , we enumerate the possible behaviors of the model in response to variation of liver insulin sensitivity and dietary glucose variability .
	manualset3
197699	6	416203	7	NULL	NULL	0	NULL	 variation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a composite model of the glucose homeostasis system , consisting of seven interconnected submodels , we enumerate the possible behaviors of the model in response to variation of liver insulin sensitivity and dietary glucose variability .
	manualset3
197700	7	416203	7	NULL	NULL	0	NULL	liver insulin sensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a composite model of the glucose homeostasis system , consisting of seven interconnected submodels , we enumerate the possible behaviors of the model in response to variation of liver insulin sensitivity and dietary glucose variability .
	manualset3
197701	8	416203	7	NULL	NULL	0	NULL	dietary glucose variability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a composite model of the glucose homeostasis system , consisting of seven interconnected submodels , we enumerate the possible behaviors of the model in response to variation of liver insulin sensitivity and dietary glucose variability .
	manualset3
197702	1	416204	7	NULL	NULL	NULL	NULL	high-sensitivity immunofluorescence procedure	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using a high-sensitivity immunofluorescence procedure , a proportion of blood lymphocytes can be shown to express the p55 chain of the IL-2 receptor ( CD25 , TAC ) without in vitro stimulation .
	manualset3
197703	2	416204	7	NULL	NULL	0	NULL	 proportion	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a high-sensitivity immunofluorescence procedure , a proportion of blood lymphocytes can be shown to express the p55 chain of the IL-2 receptor ( CD25 , TAC ) without in vitro stimulation .
	manualset3
197704	3	416204	7	NULL	NULL	0	NULL	blood lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a high-sensitivity immunofluorescence procedure , a proportion of blood lymphocytes can be shown to express the p55 chain of the IL-2 receptor ( CD25 , TAC ) without in vitro stimulation .
	manualset3
197705	4	416204	7	NULL	NULL	0	NULL	p55 chain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a high-sensitivity immunofluorescence procedure , a proportion of blood lymphocytes can be shown to express the p55 chain of the IL-2 receptor ( CD25 , TAC ) without in vitro stimulation .
	manualset3
197706	5	416204	7	NULL	NULL	0	NULL	IL-2 receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a high-sensitivity immunofluorescence procedure , a proportion of blood lymphocytes can be shown to express the p55 chain of the IL-2 receptor ( CD25 , TAC ) without in vitro stimulation .
	manualset3
197707	6	416204	7	NULL	NULL	0	NULL	CD25	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a high-sensitivity immunofluorescence procedure , a proportion of blood lymphocytes can be shown to express the p55 chain of the IL-2 receptor ( CD25 , TAC ) without in vitro stimulation .
	manualset3
197708	7	416204	7	NULL	NULL	0	NULL	 TAC	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a high-sensitivity immunofluorescence procedure , a proportion of blood lymphocytes can be shown to express the p55 chain of the IL-2 receptor ( CD25 , TAC ) without in vitro stimulation .
	manualset3
197818	8	416204	7	NULL	NULL	0	NULL	in vitro stimulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a high-sensitivity immunofluorescence procedure , a proportion of blood lymphocytes can be shown to express the p55 chain of the IL-2 receptor ( CD25 , TAC ) without in vitro stimulation .
	manualset3
197819	1	416205	7	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment and patient characteristics that confer a high risk for adverse sequelae are identified , intervention programs targeting primary or secondary interventions must be actively pursued .
	manualset3
197820	2	416205	7	NULL	NULL	0	NULL	patient characteristics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment and patient characteristics that confer a high risk for adverse sequelae are identified , intervention programs targeting primary or secondary interventions must be actively pursued .
	manualset3
197821	3	416205	7	NULL	NULL	0	NULL	high risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment and patient characteristics that confer a high risk for adverse sequelae are identified , intervention programs targeting primary or secondary interventions must be actively pursued .
	manualset3
197822	4	416205	7	NULL	NULL	0	NULL	 adverse sequelae	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment and patient characteristics that confer a high risk for adverse sequelae are identified , intervention programs targeting primary or secondary interventions must be actively pursued .
	manualset3
197823	5	416205	7	NULL	NULL	0	NULL	intervention programs	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment and patient characteristics that confer a high risk for adverse sequelae are identified , intervention programs targeting primary or secondary interventions must be actively pursued .
	manualset3
197824	6	416205	7	NULL	NULL	0	NULL	primary interventions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment and patient characteristics that confer a high risk for adverse sequelae are identified , intervention programs targeting primary or secondary interventions must be actively pursued .
	manualset3
197825	7	416205	7	NULL	NULL	0	NULL	secondary interventions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment and patient characteristics that confer a high risk for adverse sequelae are identified , intervention programs targeting primary or secondary interventions must be actively pursued .
	manualset3
197826	1	416206	7	NULL	NULL	0	NULL	human telomerase-immortalized corneal epithelial cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human telomerase-immortalized corneal epithelial cell line , IGF-1R expression and localization was assayed by immunofluorescence and subcellular fractionation followed by western blot .
	manualset3
197827	2	416206	7	NULL	NULL	0	NULL	IGF-1R expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human telomerase-immortalized corneal epithelial cell line , IGF-1R expression and localization was assayed by immunofluorescence and subcellular fractionation followed by western blot .
	manualset3
197828	3	416206	7	NULL	NULL	0	NULL	localization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human telomerase-immortalized corneal epithelial cell line , IGF-1R expression and localization was assayed by immunofluorescence and subcellular fractionation followed by western blot .
	manualset3
197829	4	416206	7	NULL	NULL	0	NULL	immunofluorescence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human telomerase-immortalized corneal epithelial cell line , IGF-1R expression and localization was assayed by immunofluorescence and subcellular fractionation followed by western blot .
	manualset3
197830	5	416206	7	NULL	NULL	0	NULL	subcellular fractionation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human telomerase-immortalized corneal epithelial cell line , IGF-1R expression and localization was assayed by immunofluorescence and subcellular fractionation followed by western blot .
	manualset3
197831	6	416206	7	NULL	NULL	0	NULL	western blot	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human telomerase-immortalized corneal epithelial cell line , IGF-1R expression and localization was assayed by immunofluorescence and subcellular fractionation followed by western blot .
	manualset3
197832	1	416207	7	NULL	NULL	0	NULL	 large set 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a large set of experimentally confirmed eukaryotic N-glycoproteins we analyzed the relative position and distribution of sequons .
	manualset3
197833	2	416207	7	NULL	NULL	0	NULL	experimentally confirmed eukaryotic N-glycoproteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a large set of experimentally confirmed eukaryotic N-glycoproteins we analyzed the relative position and distribution of sequons .
	manualset3
197834	3	416207	7	NULL	NULL	0	NULL	relative position	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a large set of experimentally confirmed eukaryotic N-glycoproteins we analyzed the relative position and distribution of sequons .
	manualset3
197835	4	416207	7	NULL	NULL	0	NULL	distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a large set of experimentally confirmed eukaryotic N-glycoproteins we analyzed the relative position and distribution of sequons .
	manualset3
197836	5	416207	7	NULL	NULL	0	NULL	sequons	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a large set of experimentally confirmed eukaryotic N-glycoproteins we analyzed the relative position and distribution of sequons .
	manualset3
197837	1	416208	7	NULL	NULL	0	NULL	mechanical search stimulus	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a mechanical search stimulus , 20 slowly and 22 rapidly adapting nasal mechanoreceptors were identified , exhibiting mean thresholds of 2.96 g. Twelve slowly adapting units also exhibited chemical sensitivity when exposed to ammonia gas .
	manualset3
197838	2	416208	7	NULL	NULL	0	NULL	 20 slowly adapting nasal mechanoreceptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a mechanical search stimulus , 20 slowly and 22 rapidly adapting nasal mechanoreceptors were identified , exhibiting mean thresholds of 2.96 g. Twelve slowly adapting units also exhibited chemical sensitivity when exposed to ammonia gas .
	manualset3
197839	3	416208	7	NULL	NULL	0	NULL	22 rapidly adapting nasal mechanoreceptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a mechanical search stimulus , 20 slowly and 22 rapidly adapting nasal mechanoreceptors were identified , exhibiting mean thresholds of 2.96 g. Twelve slowly adapting units also exhibited chemical sensitivity when exposed to ammonia gas .
	manualset3
197840	4	416208	7	NULL	NULL	0	NULL	mean thresholds	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a mechanical search stimulus , 20 slowly and 22 rapidly adapting nasal mechanoreceptors were identified , exhibiting mean thresholds of 2.96 g. Twelve slowly adapting units also exhibited chemical sensitivity when exposed to ammonia gas .
	manualset3
197841	5	416208	7	NULL	NULL	0	NULL	 2.96 g	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a mechanical search stimulus , 20 slowly and 22 rapidly adapting nasal mechanoreceptors were identified , exhibiting mean thresholds of 2.96 g. Twelve slowly adapting units also exhibited chemical sensitivity when exposed to ammonia gas .
	manualset3
197842	6	416208	7	NULL	NULL	0	NULL	Twelve slowly adapting units	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a mechanical search stimulus , 20 slowly and 22 rapidly adapting nasal mechanoreceptors were identified , exhibiting mean thresholds of 2.96 g. Twelve slowly adapting units also exhibited chemical sensitivity when exposed to ammonia gas .
	manualset3
197843	7	416208	7	NULL	NULL	0	NULL	chemical sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a mechanical search stimulus , 20 slowly and 22 rapidly adapting nasal mechanoreceptors were identified , exhibiting mean thresholds of 2.96 g. Twelve slowly adapting units also exhibited chemical sensitivity when exposed to ammonia gas .
	manualset3
197844	8	416208	7	NULL	NULL	0	NULL	ammonia gas	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a mechanical search stimulus , 20 slowly and 22 rapidly adapting nasal mechanoreceptors were identified , exhibiting mean thresholds of 2.96 g. Twelve slowly adapting units also exhibited chemical sensitivity when exposed to ammonia gas .
	manualset3
197845	1	416209	7	NULL	NULL	0	NULL	 multifunction spectrophotometer 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a multifunction spectrophotometer , the refractive index of a pigment can be estimated by measuring the backscattering of light from the pigment in immersion liquids having slightly different refractive indices .
	manualset3
197846	2	416209	7	NULL	NULL	0	NULL	 refractive index 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a multifunction spectrophotometer , the refractive index of a pigment can be estimated by measuring the backscattering of light from the pigment in immersion liquids having slightly different refractive indices .
	manualset3
197847	3	416209	7	NULL	NULL	0	NULL	pigment	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a multifunction spectrophotometer , the refractive index of a pigment can be estimated by measuring the backscattering of light from the pigment in immersion liquids having slightly different refractive indices .
	manualset3
197848	4	416209	7	NULL	NULL	0	NULL	backscattering of light	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a multifunction spectrophotometer , the refractive index of a pigment can be estimated by measuring the backscattering of light from the pigment in immersion liquids having slightly different refractive indices .
	manualset3
197849	5	416209	7	NULL	NULL	0	NULL	 pigment	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a multifunction spectrophotometer , the refractive index of a pigment can be estimated by measuring the backscattering of light from the pigment in immersion liquids having slightly different refractive indices .
	manualset3
197850	6	416209	7	NULL	NULL	0	NULL	 immersion liquids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a multifunction spectrophotometer , the refractive index of a pigment can be estimated by measuring the backscattering of light from the pigment in immersion liquids having slightly different refractive indices .
	manualset3
197851	7	416209	7	NULL	NULL	0	NULL	refractive indices	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a multifunction spectrophotometer , the refractive index of a pigment can be estimated by measuring the backscattering of light from the pigment in immersion liquids having slightly different refractive indices .
	manualset3
197852	1	416210	7	NULL	NULL	0	NULL	quality assurance audit	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a quality assurance audit .
	manualset3
198028	1	416211	7	NULL	NULL	0	NULL	radioactive in situ hybridization approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a radioactive in situ hybridization approach , the distribution of NT-2R transcripts was quantified from autoradiograms , and the cellular localization was examined in liquid emulsions .
	manualset3
198029	2	416211	7	NULL	NULL	0	NULL	 distribution 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a radioactive in situ hybridization approach , the distribution of NT-2R transcripts was quantified from autoradiograms , and the cellular localization was examined in liquid emulsions .
	manualset3
198030	3	416211	7	NULL	NULL	0	NULL	NT-2R transcripts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a radioactive in situ hybridization approach , the distribution of NT-2R transcripts was quantified from autoradiograms , and the cellular localization was examined in liquid emulsions .
	manualset3
198031	4	416211	7	NULL	NULL	0	NULL	autoradiograms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a radioactive in situ hybridization approach , the distribution of NT-2R transcripts was quantified from autoradiograms , and the cellular localization was examined in liquid emulsions .
	manualset3
198032	5	416211	7	NULL	NULL	0	NULL	cellular localization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a radioactive in situ hybridization approach , the distribution of NT-2R transcripts was quantified from autoradiograms , and the cellular localization was examined in liquid emulsions .
	manualset3
198033	6	416211	7	NULL	NULL	0	NULL	liquid emulsions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a radioactive in situ hybridization approach , the distribution of NT-2R transcripts was quantified from autoradiograms , and the cellular localization was examined in liquid emulsions .
	manualset3
198034	1	416212	7	NULL	NULL	NULL	NULL	randomly selected sample	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using a randomly selected sample of participants of Special Supplemental Nutrition Program for Women , Infants , and Children ( WIC ) in Los Angeles County , we assessed accuracy of maternal perceptions of their children 's weight status by comparing children 's weight classification to the mothers ' response to the question `` Do you consider your child to be overweight , underweight or about right weight for ( his ) ( her ) height ? ''
	manualset3
198035	2	416212	7	NULL	NULL	0	NULL	 participants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a randomly selected sample of participants of Special Supplemental Nutrition Program for Women , Infants , and Children ( WIC ) in Los Angeles County , we assessed accuracy of maternal perceptions of their children 's weight status by comparing children 's weight classification to the mothers ' response to the question `` Do you consider your child to be overweight , underweight or about right weight for ( his ) ( her ) height ? ''
	manualset3
198036	3	416212	7	NULL	NULL	0	NULL	Special Supplemental Nutrition Program for Women	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a randomly selected sample of participants of Special Supplemental Nutrition Program for Women , Infants , and Children ( WIC ) in Los Angeles County , we assessed accuracy of maternal perceptions of their children 's weight status by comparing children 's weight classification to the mothers ' response to the question `` Do you consider your child to be overweight , underweight or about right weight for ( his ) ( her ) height ? ''
	manualset3
198037	4	416212	7	NULL	NULL	0	NULL	Special Supplemental Nutrition Program for  Infants	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a randomly selected sample of participants of Special Supplemental Nutrition Program for Women , Infants , and Children ( WIC ) in Los Angeles County , we assessed accuracy of maternal perceptions of their children 's weight status by comparing children 's weight classification to the mothers ' response to the question `` Do you consider your child to be overweight , underweight or about right weight for ( his ) ( her ) height ? ''
	manualset3
198038	5	416212	7	NULL	NULL	0	NULL	Special Supplemental Nutrition Program for Children ( WIC )	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a randomly selected sample of participants of Special Supplemental Nutrition Program for Women , Infants , and Children ( WIC ) in Los Angeles County , we assessed accuracy of maternal perceptions of their children 's weight status by comparing children 's weight classification to the mothers ' response to the question `` Do you consider your child to be overweight , underweight or about right weight for ( his ) ( her ) height ? ''
	manualset3
198039	6	416212	7	NULL	NULL	0	NULL	Los Angeles County	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a randomly selected sample of participants of Special Supplemental Nutrition Program for Women , Infants , and Children ( WIC ) in Los Angeles County , we assessed accuracy of maternal perceptions of their children 's weight status by comparing children 's weight classification to the mothers ' response to the question `` Do you consider your child to be overweight , underweight or about right weight for ( his ) ( her ) height ? ''
	manualset3
198040	7	416212	7	NULL	NULL	0	NULL	maternal perceptions	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a randomly selected sample of participants of Special Supplemental Nutrition Program for Women , Infants , and Children ( WIC ) in Los Angeles County , we assessed accuracy of maternal perceptions of their children 's weight status by comparing children 's weight classification to the mothers ' response to the question `` Do you consider your child to be overweight , underweight or about right weight for ( his ) ( her ) height ? ''
	manualset3
198041	8	416212	7	NULL	NULL	0	NULL	children 's weight status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a randomly selected sample of participants of Special Supplemental Nutrition Program for Women , Infants , and Children ( WIC ) in Los Angeles County , we assessed accuracy of maternal perceptions of their children 's weight status by comparing children 's weight classification to the mothers ' response to the question `` Do you consider your child to be overweight , underweight or about right weight for ( his ) ( her ) height ? ''
	manualset3
198042	9	416212	7	NULL	NULL	0	NULL	children 's weight classification	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a randomly selected sample of participants of Special Supplemental Nutrition Program for Women , Infants , and Children ( WIC ) in Los Angeles County , we assessed accuracy of maternal perceptions of their children 's weight status by comparing children 's weight classification to the mothers ' response to the question `` Do you consider your child to be overweight , underweight or about right weight for ( his ) ( her ) height ? ''
	manualset3
198043	10	416212	7	NULL	NULL	0	NULL	mothers ' response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a randomly selected sample of participants of Special Supplemental Nutrition Program for Women , Infants , and Children ( WIC ) in Los Angeles County , we assessed accuracy of maternal perceptions of their children 's weight status by comparing children 's weight classification to the mothers ' response to the question `` Do you consider your child to be overweight , underweight or about right weight for ( his ) ( her ) height ? ''
	manualset3
198044	11	416212	7	NULL	NULL	0	NULL	question	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a randomly selected sample of participants of Special Supplemental Nutrition Program for Women , Infants , and Children ( WIC ) in Los Angeles County , we assessed accuracy of maternal perceptions of their children 's weight status by comparing children 's weight classification to the mothers ' response to the question `` Do you consider your child to be overweight , underweight or about right weight for ( his ) ( her ) height ? ''
	manualset3
198045	12	416212	7	NULL	NULL	NULL	NULL	 child 	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using a randomly selected sample of participants of Special Supplemental Nutrition Program for Women , Infants , and Children ( WIC ) in Los Angeles County , we assessed accuracy of maternal perceptions of their children 's weight status by comparing children 's weight classification to the mothers ' response to the question `` Do you consider your child to be overweight , underweight or about right weight for ( his ) ( her ) height ? ''
	manualset3
203074	13	416212	7	NULL	NULL	0	NULL	overweight 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a randomly selected sample of participants of Special Supplemental Nutrition Program for Women , Infants , and Children ( WIC ) in Los Angeles County , we assessed accuracy of maternal perceptions of their children 's weight status by comparing children 's weight classification to the mothers ' response to the question `` Do you consider your child to be overweight , underweight or about right weight for ( his ) ( her ) height ? ''
	manualset3
203075	14	416212	7	NULL	NULL	0	NULL	underweight	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a randomly selected sample of participants of Special Supplemental Nutrition Program for Women , Infants , and Children ( WIC ) in Los Angeles County , we assessed accuracy of maternal perceptions of their children 's weight status by comparing children 's weight classification to the mothers ' response to the question `` Do you consider your child to be overweight , underweight or about right weight for ( his ) ( her ) height ? ''
	manualset3
203076	15	416212	7	NULL	NULL	0	NULL	 right weight	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a randomly selected sample of participants of Special Supplemental Nutrition Program for Women , Infants , and Children ( WIC ) in Los Angeles County , we assessed accuracy of maternal perceptions of their children 's weight status by comparing children 's weight classification to the mothers ' response to the question `` Do you consider your child to be overweight , underweight or about right weight for ( his ) ( her ) height ? ''
	manualset3
203077	16	416212	7	NULL	NULL	0	NULL	 height	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a randomly selected sample of participants of Special Supplemental Nutrition Program for Women , Infants , and Children ( WIC ) in Los Angeles County , we assessed accuracy of maternal perceptions of their children 's weight status by comparing children 's weight classification to the mothers ' response to the question `` Do you consider your child to be overweight , underweight or about right weight for ( his ) ( her ) height ? ''
	manualset3
203078	17	416212	7	NULL	NULL	0	NULL	accuracy 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a randomly selected sample of participants of Special Supplemental Nutrition Program for Women , Infants , and Children ( WIC ) in Los Angeles County , we assessed accuracy of maternal perceptions of their children 's weight status by comparing children 's weight classification to the mothers ' response to the question `` Do you consider your child to be overweight , underweight or about right weight for ( his ) ( her ) height ? ''
	manualset3
203079	18	416212	7	NULL	NULL	NULL	NULL	comparing	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using a randomly selected sample of participants of Special Supplemental Nutrition Program for Women , Infants , and Children ( WIC ) in Los Angeles County , we assessed accuracy of maternal perceptions of their children 's weight status by comparing children 's weight classification to the mothers ' response to the question `` Do you consider your child to be overweight , underweight or about right weight for ( his ) ( her ) height ? ''
	manualset3
198046	1	416213	7	NULL	NULL	0	NULL	renaturation kinase assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a renaturation kinase assay , we demonstrated that pp43 is capable of autophosphorylation on serine and threonine , thus identifying it as a new protein serine/threonine kinase .
	manualset3
198047	2	416213	7	NULL	NULL	0	NULL	pp43	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a renaturation kinase assay , we demonstrated that pp43 is capable of autophosphorylation on serine and threonine , thus identifying it as a new protein serine/threonine kinase .
	manualset3
198048	3	416213	7	NULL	NULL	0	NULL	autophosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a renaturation kinase assay , we demonstrated that pp43 is capable of autophosphorylation on serine and threonine , thus identifying it as a new protein serine/threonine kinase .
	manualset3
198049	4	416213	7	NULL	NULL	0	NULL	serine 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a renaturation kinase assay , we demonstrated that pp43 is capable of autophosphorylation on serine and threonine , thus identifying it as a new protein serine/threonine kinase .
	manualset3
198050	5	416213	7	NULL	NULL	0	NULL	threonine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a renaturation kinase assay , we demonstrated that pp43 is capable of autophosphorylation on serine and threonine , thus identifying it as a new protein serine/threonine kinase .
	manualset3
198051	6	416213	7	NULL	NULL	0	NULL	new protein serine/threonine kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a renaturation kinase assay , we demonstrated that pp43 is capable of autophosphorylation on serine and threonine , thus identifying it as a new protein serine/threonine kinase .
	manualset3
198052	1	416214	7	NULL	NULL	0	NULL	 treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment fear of flying was significantly reduced .
	manualset3
198053	2	416214	7	NULL	NULL	0	NULL	fear of flying	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment fear of flying was significantly reduced .
	manualset3
198054	1	416215	7	NULL	NULL	0	NULL	soluble TREM-1 fusion protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a soluble TREM-1 fusion protein , we demonstrate that after intravenous injection of LPS TREM-1L was induced on Gr-1 ( + ) granulocytes and monocytes but not on other cell populations in peripheral blood .
	manualset3
198055	2	416215	7	NULL	NULL	0	NULL	intravenous injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a soluble TREM-1 fusion protein , we demonstrate that after intravenous injection of LPS TREM-1L was induced on Gr-1 ( + ) granulocytes and monocytes but not on other cell populations in peripheral blood .
	manualset3
198056	3	416215	7	NULL	NULL	0	NULL	LPS TREM-1L	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a soluble TREM-1 fusion protein , we demonstrate that after intravenous injection of LPS TREM-1L was induced on Gr-1 ( + ) granulocytes and monocytes but not on other cell populations in peripheral blood .
	manualset3
198057	4	416215	7	NULL	NULL	0	NULL	Gr-1 ( + ) granulocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a soluble TREM-1 fusion protein , we demonstrate that after intravenous injection of LPS TREM-1L was induced on Gr-1 ( + ) granulocytes and monocytes but not on other cell populations in peripheral blood .
	manualset3
198058	5	416215	7	NULL	NULL	0	NULL	monocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a soluble TREM-1 fusion protein , we demonstrate that after intravenous injection of LPS TREM-1L was induced on Gr-1 ( + ) granulocytes and monocytes but not on other cell populations in peripheral blood .
	manualset3
198059	6	416215	7	NULL	NULL	0	NULL	cell populations	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a soluble TREM-1 fusion protein , we demonstrate that after intravenous injection of LPS TREM-1L was induced on Gr-1 ( + ) granulocytes and monocytes but not on other cell populations in peripheral blood .
	manualset3
198060	7	416215	7	NULL	NULL	0	NULL	 peripheral blood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a soluble TREM-1 fusion protein , we demonstrate that after intravenous injection of LPS TREM-1L was induced on Gr-1 ( + ) granulocytes and monocytes but not on other cell populations in peripheral blood .
	manualset3
198061	1	416216	7	NULL	NULL	0	NULL	 stochastic model	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a stochastic model , we show that the pattern of cell death of striatal neurons might contribute up to 20 % of variance of AO .
	manualset3
198062	2	416216	7	NULL	NULL	0	NULL	pattern of cell death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a stochastic model , we show that the pattern of cell death of striatal neurons might contribute up to 20 % of variance of AO .
	manualset3
198063	3	416216	7	NULL	NULL	0	NULL	 striatal neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a stochastic model , we show that the pattern of cell death of striatal neurons might contribute up to 20 % of variance of AO .
	manualset3
198064	4	416216	7	NULL	NULL	0	NULL	20 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a stochastic model , we show that the pattern of cell death of striatal neurons might contribute up to 20 % of variance of AO .
	manualset3
198065	5	416216	7	NULL	NULL	0	NULL	variance	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a stochastic model , we show that the pattern of cell death of striatal neurons might contribute up to 20 % of variance of AO .
	manualset3
198066	6	416216	7	NULL	NULL	0	NULL	AO	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a stochastic model , we show that the pattern of cell death of striatal neurons might contribute up to 20 % of variance of AO .
	manualset3
198067	1	416217	7	NULL	NULL	0	NULL	 absorption  fluorescence spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using absorption , steady-state and time-resolved fluorescence spectroscopy , dynamic light scattering , and cysteine accessibility studies , tertiary structure of denatured states was characterized .
	manualset3
198068	2	416217	7	NULL	NULL	0	NULL	 steady-state and time-resolved fluorescence spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using absorption , steady-state and time-resolved fluorescence spectroscopy , dynamic light scattering , and cysteine accessibility studies , tertiary structure of denatured states was characterized .
	manualset3
198069	3	416217	7	NULL	NULL	0	NULL	 dynamic light scattering	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using absorption , steady-state and time-resolved fluorescence spectroscopy , dynamic light scattering , and cysteine accessibility studies , tertiary structure of denatured states was characterized .
	manualset3
198070	4	416217	7	NULL	NULL	0	NULL	cysteine accessibility studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using absorption , steady-state and time-resolved fluorescence spectroscopy , dynamic light scattering , and cysteine accessibility studies , tertiary structure of denatured states was characterized .
	manualset3
198071	5	416217	7	NULL	NULL	0	NULL	tertiary structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using absorption , steady-state and time-resolved fluorescence spectroscopy , dynamic light scattering , and cysteine accessibility studies , tertiary structure of denatured states was characterized .
	manualset3
198072	6	416217	7	NULL	NULL	0	NULL	denatured states 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using absorption , steady-state and time-resolved fluorescence spectroscopy , dynamic light scattering , and cysteine accessibility studies , tertiary structure of denatured states was characterized .
	manualset3
198073	1	416218	7	NULL	NULL	0	NULL	acetone fractionation electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using acetone fractionation and a subsequent preparative electrophoresis in a phenol solution , protein P-9 was isolated from the nuclei of lymphoma NK/Ly and Gerene carcinoma in a pure state .
	manualset3
198074	2	416218	7	NULL	NULL	0	NULL	subsequent preparative electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using acetone fractionation and a subsequent preparative electrophoresis in a phenol solution , protein P-9 was isolated from the nuclei of lymphoma NK/Ly and Gerene carcinoma in a pure state .
	manualset3
198075	3	416218	7	NULL	NULL	0	NULL	phenol solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using acetone fractionation and a subsequent preparative electrophoresis in a phenol solution , protein P-9 was isolated from the nuclei of lymphoma NK/Ly and Gerene carcinoma in a pure state .
	manualset3
198076	4	416218	7	NULL	NULL	0	NULL	protein P-9	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using acetone fractionation and a subsequent preparative electrophoresis in a phenol solution , protein P-9 was isolated from the nuclei of lymphoma NK/Ly and Gerene carcinoma in a pure state .
	manualset3
198077	5	416218	7	NULL	NULL	0	NULL	nuclei	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Using acetone fractionation and a subsequent preparative electrophoresis in a phenol solution , protein P-9 was isolated from the nuclei of lymphoma NK/Ly and Gerene carcinoma in a pure state .
	manualset3
198078	6	416218	7	NULL	NULL	0	NULL	lymphoma NK/Ly	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Using acetone fractionation and a subsequent preparative electrophoresis in a phenol solution , protein P-9 was isolated from the nuclei of lymphoma NK/Ly and Gerene carcinoma in a pure state .
	manualset3
198079	7	416218	7	NULL	NULL	0	NULL	Gerene carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Using acetone fractionation and a subsequent preparative electrophoresis in a phenol solution , protein P-9 was isolated from the nuclei of lymphoma NK/Ly and Gerene carcinoma in a pure state .
	manualset3
198080	8	416218	7	NULL	NULL	NULL	NULL	pure state 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using acetone fractionation and a subsequent preparative electrophoresis in a phenol solution , protein P-9 was isolated from the nuclei of lymphoma NK/Ly and Gerene carcinoma in a pure state .
	manualset3
198081	1	416219	7	NULL	NULL	0	NULL	amplification	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using amplification of genomic DNA and flow-sorted chromosomes we have assigned the gene ( LAMA4 ) for this new laminin A variant to chromosome 6 .
	manualset3
198082	2	416219	7	NULL	NULL	0	NULL	 genomic DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using amplification of genomic DNA and flow-sorted chromosomes we have assigned the gene ( LAMA4 ) for this new laminin A variant to chromosome 6 .
	manualset3
198083	3	416219	7	NULL	NULL	0	NULL	 flow-sorted chromosomes	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Using amplification of genomic DNA and flow-sorted chromosomes we have assigned the gene ( LAMA4 ) for this new laminin A variant to chromosome 6 .
	manualset3
198084	4	416219	7	NULL	NULL	0	NULL	gene ( LAMA4 )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Using amplification of genomic DNA and flow-sorted chromosomes we have assigned the gene ( LAMA4 ) for this new laminin A variant to chromosome 6 .
	manualset3
198085	5	416219	7	NULL	NULL	0	NULL	laminin A variant	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Using amplification of genomic DNA and flow-sorted chromosomes we have assigned the gene ( LAMA4 ) for this new laminin A variant to chromosome 6 .
	manualset3
198086	6	416219	7	NULL	NULL	0	NULL	chromosome 6	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Using amplification of genomic DNA and flow-sorted chromosomes we have assigned the gene ( LAMA4 ) for this new laminin A variant to chromosome 6 .
	manualset3
198087	1	416220	7	NULL	NULL	0	NULL	skeletal-muscle fractionation procedure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an established skeletal-muscle fractionation procedure we present evidence for the existence of two distinct intracellular GLUT4 compartments .
	manualset3
198088	2	416220	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an established skeletal-muscle fractionation procedure we present evidence for the existence of two distinct intracellular GLUT4 compartments .
	manualset3
198089	3	416220	7	NULL	NULL	0	NULL	existence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an established skeletal-muscle fractionation procedure we present evidence for the existence of two distinct intracellular GLUT4 compartments .
	manualset3
198090	4	416220	7	NULL	NULL	0	NULL	two distinct intracellular GLUT4 compartments	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an established skeletal-muscle fractionation procedure we present evidence for the existence of two distinct intracellular GLUT4 compartments .
	manualset3
198091	1	416221	7	NULL	NULL	0	NULL	experimental model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an experimental model of autologous BMT , recipients of 10 ( 3 ) tumor cells could also be cured following transplantation of syngeneic spleen cells by high-dose IL-2 ( 10 ( 5 ) U x 3/day x 5 days ) given at the time lymphocytes were present , optimally at 3 weeks following BMT .
	manualset3
198092	2	416221	7	NULL	NULL	0	NULL	autologous BMT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an experimental model of autologous BMT , recipients of 10 ( 3 ) tumor cells could also be cured following transplantation of syngeneic spleen cells by high-dose IL-2 ( 10 ( 5 ) U x 3/day x 5 days ) given at the time lymphocytes were present , optimally at 3 weeks following BMT .
	manualset3
198093	3	416221	7	NULL	NULL	0	NULL	recipients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an experimental model of autologous BMT , recipients of 10 ( 3 ) tumor cells could also be cured following transplantation of syngeneic spleen cells by high-dose IL-2 ( 10 ( 5 ) U x 3/day x 5 days ) given at the time lymphocytes were present , optimally at 3 weeks following BMT .
	manualset3
198094	4	416221	7	NULL	NULL	0	NULL	10 ( 3 ) tumor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an experimental model of autologous BMT , recipients of 10 ( 3 ) tumor cells could also be cured following transplantation of syngeneic spleen cells by high-dose IL-2 ( 10 ( 5 ) U x 3/day x 5 days ) given at the time lymphocytes were present , optimally at 3 weeks following BMT .
	manualset3
198095	5	416221	7	NULL	NULL	0	NULL	transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an experimental model of autologous BMT , recipients of 10 ( 3 ) tumor cells could also be cured following transplantation of syngeneic spleen cells by high-dose IL-2 ( 10 ( 5 ) U x 3/day x 5 days ) given at the time lymphocytes were present , optimally at 3 weeks following BMT .
	manualset3
198096	6	416221	7	NULL	NULL	0	NULL	syngeneic spleen cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an experimental model of autologous BMT , recipients of 10 ( 3 ) tumor cells could also be cured following transplantation of syngeneic spleen cells by high-dose IL-2 ( 10 ( 5 ) U x 3/day x 5 days ) given at the time lymphocytes were present , optimally at 3 weeks following BMT .
	manualset3
198097	7	416221	7	NULL	NULL	0	NULL	high-dose IL-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an experimental model of autologous BMT , recipients of 10 ( 3 ) tumor cells could also be cured following transplantation of syngeneic spleen cells by high-dose IL-2 ( 10 ( 5 ) U x 3/day x 5 days ) given at the time lymphocytes were present , optimally at 3 weeks following BMT .
	manualset3
198098	8	416221	7	NULL	NULL	0	NULL	( 10 ( 5 ) U x 3/day x 5 days )	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an experimental model of autologous BMT , recipients of 10 ( 3 ) tumor cells could also be cured following transplantation of syngeneic spleen cells by high-dose IL-2 ( 10 ( 5 ) U x 3/day x 5 days ) given at the time lymphocytes were present , optimally at 3 weeks following BMT .
	manualset3
198099	9	416221	7	NULL	NULL	0	NULL	 time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an experimental model of autologous BMT , recipients of 10 ( 3 ) tumor cells could also be cured following transplantation of syngeneic spleen cells by high-dose IL-2 ( 10 ( 5 ) U x 3/day x 5 days ) given at the time lymphocytes were present , optimally at 3 weeks following BMT .
	manualset3
198100	10	416221	7	NULL	NULL	0	NULL	 lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an experimental model of autologous BMT , recipients of 10 ( 3 ) tumor cells could also be cured following transplantation of syngeneic spleen cells by high-dose IL-2 ( 10 ( 5 ) U x 3/day x 5 days ) given at the time lymphocytes were present , optimally at 3 weeks following BMT .
	manualset3
198101	11	416221	7	NULL	NULL	0	NULL	3 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an experimental model of autologous BMT , recipients of 10 ( 3 ) tumor cells could also be cured following transplantation of syngeneic spleen cells by high-dose IL-2 ( 10 ( 5 ) U x 3/day x 5 days ) given at the time lymphocytes were present , optimally at 3 weeks following BMT .
	manualset3
198102	12	416221	7	NULL	NULL	0	NULL	BMT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an experimental model of autologous BMT , recipients of 10 ( 3 ) tumor cells could also be cured following transplantation of syngeneic spleen cells by high-dose IL-2 ( 10 ( 5 ) U x 3/day x 5 days ) given at the time lymphocytes were present , optimally at 3 weeks following BMT .
	manualset3
198103	1	416222	7	NULL	NULL	NULL	NULL	in vitro column perifusion system	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using an in vitro column perifusion system , a superactive gonadotropin-releasing hormone ( GnRH ) analog ( d-Arg6 , Pro9-NEt ) - sGnRH ( sGnRHa , 0.3-30 nM ) , dopamine ( DA , 0.1-10 muM ) , and the nonselective DA agonist apomorphine ( 0.1-10 muM ) stimulated GH release from grass carp pituitary cells in a dose-dependent manner .
	manualset3
198104	2	416222	7	NULL	NULL	0	NULL	superactive gonadotropin-releasing hormone ( GnRH ) analog ( d-Arg6 , Pro9-NEt ) - sGnRH	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an in vitro column perifusion system , a superactive gonadotropin-releasing hormone ( GnRH ) analog ( d-Arg6 , Pro9-NEt ) - sGnRH ( sGnRHa , 0.3-30 nM ) , dopamine ( DA , 0.1-10 muM ) , and the nonselective DA agonist apomorphine ( 0.1-10 muM ) stimulated GH release from grass carp pituitary cells in a dose-dependent manner .
	manualset3
198105	3	416222	7	NULL	NULL	0	NULL	sGnRHa	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an in vitro column perifusion system , a superactive gonadotropin-releasing hormone ( GnRH ) analog ( d-Arg6 , Pro9-NEt ) - sGnRH ( sGnRHa , 0.3-30 nM ) , dopamine ( DA , 0.1-10 muM ) , and the nonselective DA agonist apomorphine ( 0.1-10 muM ) stimulated GH release from grass carp pituitary cells in a dose-dependent manner .
	manualset3
198106	4	416222	7	NULL	NULL	NULL	NULL	0.3-30 nM	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using an in vitro column perifusion system , a superactive gonadotropin-releasing hormone ( GnRH ) analog ( d-Arg6 , Pro9-NEt ) - sGnRH ( sGnRHa , 0.3-30 nM ) , dopamine ( DA , 0.1-10 muM ) , and the nonselective DA agonist apomorphine ( 0.1-10 muM ) stimulated GH release from grass carp pituitary cells in a dose-dependent manner .
	manualset3
198107	5	416222	7	NULL	NULL	0	NULL	dopamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an in vitro column perifusion system , a superactive gonadotropin-releasing hormone ( GnRH ) analog ( d-Arg6 , Pro9-NEt ) - sGnRH ( sGnRHa , 0.3-30 nM ) , dopamine ( DA , 0.1-10 muM ) , and the nonselective DA agonist apomorphine ( 0.1-10 muM ) stimulated GH release from grass carp pituitary cells in a dose-dependent manner .
	manualset3
198108	6	416222	7	NULL	NULL	0	NULL	DA , 0.1-10 muM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an in vitro column perifusion system , a superactive gonadotropin-releasing hormone ( GnRH ) analog ( d-Arg6 , Pro9-NEt ) - sGnRH ( sGnRHa , 0.3-30 nM ) , dopamine ( DA , 0.1-10 muM ) , and the nonselective DA agonist apomorphine ( 0.1-10 muM ) stimulated GH release from grass carp pituitary cells in a dose-dependent manner .
	manualset3
198109	7	416222	7	NULL	NULL	0	NULL	nonselective DA agonist apomorphine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an in vitro column perifusion system , a superactive gonadotropin-releasing hormone ( GnRH ) analog ( d-Arg6 , Pro9-NEt ) - sGnRH ( sGnRHa , 0.3-30 nM ) , dopamine ( DA , 0.1-10 muM ) , and the nonselective DA agonist apomorphine ( 0.1-10 muM ) stimulated GH release from grass carp pituitary cells in a dose-dependent manner .
	manualset3
198110	8	416222	7	NULL	NULL	0	NULL	0.1-10 muM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an in vitro column perifusion system , a superactive gonadotropin-releasing hormone ( GnRH ) analog ( d-Arg6 , Pro9-NEt ) - sGnRH ( sGnRHa , 0.3-30 nM ) , dopamine ( DA , 0.1-10 muM ) , and the nonselective DA agonist apomorphine ( 0.1-10 muM ) stimulated GH release from grass carp pituitary cells in a dose-dependent manner .
	manualset3
198111	9	416222	7	NULL	NULL	NULL	NULL	GH release	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using an in vitro column perifusion system , a superactive gonadotropin-releasing hormone ( GnRH ) analog ( d-Arg6 , Pro9-NEt ) - sGnRH ( sGnRHa , 0.3-30 nM ) , dopamine ( DA , 0.1-10 muM ) , and the nonselective DA agonist apomorphine ( 0.1-10 muM ) stimulated GH release from grass carp pituitary cells in a dose-dependent manner .
	manualset3
198112	10	416222	7	NULL	NULL	0	NULL	grass carp pituitary cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an in vitro column perifusion system , a superactive gonadotropin-releasing hormone ( GnRH ) analog ( d-Arg6 , Pro9-NEt ) - sGnRH ( sGnRHa , 0.3-30 nM ) , dopamine ( DA , 0.1-10 muM ) , and the nonselective DA agonist apomorphine ( 0.1-10 muM ) stimulated GH release from grass carp pituitary cells in a dose-dependent manner .
	manualset3
198113	11	416222	7	NULL	NULL	0	NULL	dose-dependent manner	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an in vitro column perifusion system , a superactive gonadotropin-releasing hormone ( GnRH ) analog ( d-Arg6 , Pro9-NEt ) - sGnRH ( sGnRHa , 0.3-30 nM ) , dopamine ( DA , 0.1-10 muM ) , and the nonselective DA agonist apomorphine ( 0.1-10 muM ) stimulated GH release from grass carp pituitary cells in a dose-dependent manner .
	manualset3
198114	1	416223	7	NULL	NULL	0	NULL	in vitro kinase assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an in vitro kinase assay targeting SIK2 , we identified fisetin as a candidate inhibitor , possibly being capable of promoting melanogenesis .
	manualset3
198115	2	416223	7	NULL	NULL	0	NULL	SIK2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an in vitro kinase assay targeting SIK2 , we identified fisetin as a candidate inhibitor , possibly being capable of promoting melanogenesis .
	manualset3
198116	3	416223	7	NULL	NULL	0	NULL	fisetin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an in vitro kinase assay targeting SIK2 , we identified fisetin as a candidate inhibitor , possibly being capable of promoting melanogenesis .
	manualset3
198117	4	416223	7	NULL	NULL	0	NULL	candidate inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an in vitro kinase assay targeting SIK2 , we identified fisetin as a candidate inhibitor , possibly being capable of promoting melanogenesis .
	manualset3
198118	5	416223	7	NULL	NULL	0	NULL	melanogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an in vitro kinase assay targeting SIK2 , we identified fisetin as a candidate inhibitor , possibly being capable of promoting melanogenesis .
	manualset3
198119	1	416224	7	NULL	NULL	0	NULL	 treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment for breast cancer , many women experience cognitive problems , as determined by objective neuropsychological tests .
	manualset3
198120	2	416224	7	NULL	NULL	0	NULL	breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment for breast cancer , many women experience cognitive problems , as determined by objective neuropsychological tests .
	manualset3
198121	3	416224	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment for breast cancer , many women experience cognitive problems , as determined by objective neuropsychological tests .
	manualset3
198122	4	416224	7	NULL	NULL	0	NULL	cognitive problems	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment for breast cancer , many women experience cognitive problems , as determined by objective neuropsychological tests .
	manualset3
198123	5	416224	7	NULL	NULL	0	NULL	 objective neuropsychological tests	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment for breast cancer , many women experience cognitive problems , as determined by objective neuropsychological tests .
	manualset3
198124	1	416225	7	NULL	NULL	0	NULL	iterative linear least-squares method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an iterative linear least-squares method that decomposes water and fat images from source images acquired at short TE increments , images with a high signal-to-noise ratio ( SNR ) and uniform separation of water and fat are obtained .
	manualset3
198125	2	416225	7	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an iterative linear least-squares method that decomposes water and fat images from source images acquired at short TE increments , images with a high signal-to-noise ratio ( SNR ) and uniform separation of water and fat are obtained .
	manualset3
198126	3	416225	7	NULL	NULL	0	NULL	fat images	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an iterative linear least-squares method that decomposes water and fat images from source images acquired at short TE increments , images with a high signal-to-noise ratio ( SNR ) and uniform separation of water and fat are obtained .
	manualset3
198127	4	416225	7	NULL	NULL	0	NULL	source images	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an iterative linear least-squares method that decomposes water and fat images from source images acquired at short TE increments , images with a high signal-to-noise ratio ( SNR ) and uniform separation of water and fat are obtained .
	manualset3
198128	5	416225	7	NULL	NULL	0	NULL	short TE increments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an iterative linear least-squares method that decomposes water and fat images from source images acquired at short TE increments , images with a high signal-to-noise ratio ( SNR ) and uniform separation of water and fat are obtained .
	manualset3
198129	6	416225	7	NULL	NULL	0	NULL	 images	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an iterative linear least-squares method that decomposes water and fat images from source images acquired at short TE increments , images with a high signal-to-noise ratio ( SNR ) and uniform separation of water and fat are obtained .
	manualset3
198130	7	416225	7	NULL	NULL	0	NULL	high signal-to-noise ratio ( SNR ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an iterative linear least-squares method that decomposes water and fat images from source images acquired at short TE increments , images with a high signal-to-noise ratio ( SNR ) and uniform separation of water and fat are obtained .
	manualset3
198131	8	416225	7	NULL	NULL	0	NULL	uniform separation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an iterative linear least-squares method that decomposes water and fat images from source images acquired at short TE increments , images with a high signal-to-noise ratio ( SNR ) and uniform separation of water and fat are obtained .
	manualset3
198132	9	416225	7	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an iterative linear least-squares method that decomposes water and fat images from source images acquired at short TE increments , images with a high signal-to-noise ratio ( SNR ) and uniform separation of water and fat are obtained .
	manualset3
198133	10	416225	7	NULL	NULL	0	NULL	 fat 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using an iterative linear least-squares method that decomposes water and fat images from source images acquired at short TE increments , images with a high signal-to-noise ratio ( SNR ) and uniform separation of water and fat are obtained .
	manualset3
198134	1	416226	7	NULL	NULL	0	NULL	atomic force microscopy ( AFM )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using atomic force microscopy ( AFM ) , coupled with biochemical techniques , we demonstrate that adenine nucleotides induce large asymmetric conformational changes in full-length yeast and human MutL alpha and that these changes are associated with significant increases in secondary structure .
	manualset3
198135	2	416226	7	NULL	NULL	0	NULL	biochemical techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using atomic force microscopy ( AFM ) , coupled with biochemical techniques , we demonstrate that adenine nucleotides induce large asymmetric conformational changes in full-length yeast and human MutL alpha and that these changes are associated with significant increases in secondary structure .
	manualset3
198136	3	416226	7	NULL	NULL	0	NULL	adenine nucleotides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using atomic force microscopy ( AFM ) , coupled with biochemical techniques , we demonstrate that adenine nucleotides induce large asymmetric conformational changes in full-length yeast and human MutL alpha and that these changes are associated with significant increases in secondary structure .
	manualset3
198137	4	416226	7	NULL	NULL	0	NULL	 large asymmetric conformational changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using atomic force microscopy ( AFM ) , coupled with biochemical techniques , we demonstrate that adenine nucleotides induce large asymmetric conformational changes in full-length yeast and human MutL alpha and that these changes are associated with significant increases in secondary structure .
	manualset3
198138	5	416226	7	NULL	NULL	0	NULL	full-length yeast 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Using atomic force microscopy ( AFM ) , coupled with biochemical techniques , we demonstrate that adenine nucleotides induce large asymmetric conformational changes in full-length yeast and human MutL alpha and that these changes are associated with significant increases in secondary structure .
	manualset3
198139	6	416226	7	NULL	NULL	0	NULL	human MutL alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using atomic force microscopy ( AFM ) , coupled with biochemical techniques , we demonstrate that adenine nucleotides induce large asymmetric conformational changes in full-length yeast and human MutL alpha and that these changes are associated with significant increases in secondary structure .
	manualset3
198140	7	416226	7	NULL	NULL	0	NULL	changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using atomic force microscopy ( AFM ) , coupled with biochemical techniques , we demonstrate that adenine nucleotides induce large asymmetric conformational changes in full-length yeast and human MutL alpha and that these changes are associated with significant increases in secondary structure .
	manualset3
198141	8	416226	7	NULL	NULL	0	NULL	 secondary structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using atomic force microscopy ( AFM ) , coupled with biochemical techniques , we demonstrate that adenine nucleotides induce large asymmetric conformational changes in full-length yeast and human MutL alpha and that these changes are associated with significant increases in secondary structure .
	manualset3
198142	1	416227	7	NULL	NULL	0	NULL	bisulfite genomic sequencing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using bisulfite genomic sequencing , we have assessed the methylation status of cytosine ( including 154 CpG sites ) in six CpG-rich regions of the human IGF2-H19 genes .
	manualset3
198143	2	416227	7	NULL	NULL	0	NULL	methylation status	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using bisulfite genomic sequencing , we have assessed the methylation status of cytosine ( including 154 CpG sites ) in six CpG-rich regions of the human IGF2-H19 genes .
	manualset3
198144	3	416227	7	NULL	NULL	0	NULL	cytosine	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using bisulfite genomic sequencing , we have assessed the methylation status of cytosine ( including 154 CpG sites ) in six CpG-rich regions of the human IGF2-H19 genes .
	manualset3
198145	4	416227	7	NULL	NULL	0	NULL	154 CpG sites	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using bisulfite genomic sequencing , we have assessed the methylation status of cytosine ( including 154 CpG sites ) in six CpG-rich regions of the human IGF2-H19 genes .
	manualset3
198146	5	416227	7	NULL	NULL	0	NULL	six CpG-rich regions	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using bisulfite genomic sequencing , we have assessed the methylation status of cytosine ( including 154 CpG sites ) in six CpG-rich regions of the human IGF2-H19 genes .
	manualset3
198147	6	416227	7	NULL	NULL	0	NULL	human IGF2-H19 genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using bisulfite genomic sequencing , we have assessed the methylation status of cytosine ( including 154 CpG sites ) in six CpG-rich regions of the human IGF2-H19 genes .
	manualset3
198148	1	416228	7	NULL	NULL	0	NULL	cDNA clones 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using cDNA clones corresponding to four of the different forms of LCA molecules , extracellular domains of the LCA molecules were synthesized in vitro .
	manualset3
198149	2	416228	7	NULL	NULL	0	NULL	 four	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using cDNA clones corresponding to four of the different forms of LCA molecules , extracellular domains of the LCA molecules were synthesized in vitro .
	manualset3
198150	3	416228	7	NULL	NULL	0	NULL	different forms	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Using cDNA clones corresponding to four of the different forms of LCA molecules , extracellular domains of the LCA molecules were synthesized in vitro .
	manualset3
198151	4	416228	7	NULL	NULL	0	NULL	LCA molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Using cDNA clones corresponding to four of the different forms of LCA molecules , extracellular domains of the LCA molecules were synthesized in vitro .
	manualset3
198152	5	416228	7	NULL	NULL	0	NULL	extracellular domains 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using cDNA clones corresponding to four of the different forms of LCA molecules , extracellular domains of the LCA molecules were synthesized in vitro .
	manualset3
198153	6	416228	7	NULL	NULL	0	NULL	LCA molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Using cDNA clones corresponding to four of the different forms of LCA molecules , extracellular domains of the LCA molecules were synthesized in vitro .
	manualset3
198154	1	416229	7	NULL	NULL	0	NULL	calcium-free culture conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Using calcium-free culture conditions or the specific inhibitor of ERK phosphorylation ( UO126 ) , we demonstrated that Pi effects on Glvr-1 and -2 up-regulation require the presence of calcium and involve ERK signalling pathways .
	manualset3
198155	2	416229	7	NULL	NULL	0	NULL	specific inhibitor of ERK phosphorylation ( UO126 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using calcium-free culture conditions or the specific inhibitor of ERK phosphorylation ( UO126 ) , we demonstrated that Pi effects on Glvr-1 and -2 up-regulation require the presence of calcium and involve ERK signalling pathways .
	manualset3
198156	3	416229	7	NULL	NULL	0	NULL	Pi effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using calcium-free culture conditions or the specific inhibitor of ERK phosphorylation ( UO126 ) , we demonstrated that Pi effects on Glvr-1 and -2 up-regulation require the presence of calcium and involve ERK signalling pathways .
	manualset3
198157	4	416229	7	NULL	NULL	0	NULL	Glvr-1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using calcium-free culture conditions or the specific inhibitor of ERK phosphorylation ( UO126 ) , we demonstrated that Pi effects on Glvr-1 and -2 up-regulation require the presence of calcium and involve ERK signalling pathways .
	manualset3
198158	5	416229	7	NULL	NULL	0	NULL	Glvr-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using calcium-free culture conditions or the specific inhibitor of ERK phosphorylation ( UO126 ) , we demonstrated that Pi effects on Glvr-1 and -2 up-regulation require the presence of calcium and involve ERK signalling pathways .
	manualset3
198159	6	416229	7	NULL	NULL	0	NULL	up-regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using calcium-free culture conditions or the specific inhibitor of ERK phosphorylation ( UO126 ) , we demonstrated that Pi effects on Glvr-1 and -2 up-regulation require the presence of calcium and involve ERK signalling pathways .
	manualset3
198160	7	416229	7	NULL	NULL	0	NULL	calcium 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using calcium-free culture conditions or the specific inhibitor of ERK phosphorylation ( UO126 ) , we demonstrated that Pi effects on Glvr-1 and -2 up-regulation require the presence of calcium and involve ERK signalling pathways .
	manualset3
198161	8	416229	7	NULL	NULL	0	NULL	ERK signalling pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using calcium-free culture conditions or the specific inhibitor of ERK phosphorylation ( UO126 ) , we demonstrated that Pi effects on Glvr-1 and -2 up-regulation require the presence of calcium and involve ERK signalling pathways .
	manualset3
198162	1	416230	7	NULL	NULL	0	NULL	chimeras	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using chimeras of c-Jun and EB1 , we demonstrate that a 12 amino acid region in the basic region of the c-Jun DNA-binding domain is essential for repression by E1A .
	manualset3
198163	2	416230	7	NULL	NULL	NULL	NULL	c-Jun	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using chimeras of c-Jun and EB1 , we demonstrate that a 12 amino acid region in the basic region of the c-Jun DNA-binding domain is essential for repression by E1A .
	manualset3
198164	3	416230	7	NULL	NULL	NULL	NULL	EB1	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using chimeras of c-Jun and EB1 , we demonstrate that a 12 amino acid region in the basic region of the c-Jun DNA-binding domain is essential for repression by E1A .
	manualset3
198165	4	416230	7	NULL	NULL	0	NULL	12 amino acid region 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using chimeras of c-Jun and EB1 , we demonstrate that a 12 amino acid region in the basic region of the c-Jun DNA-binding domain is essential for repression by E1A .
	manualset3
198166	5	416230	7	NULL	NULL	0	NULL	basic region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using chimeras of c-Jun and EB1 , we demonstrate that a 12 amino acid region in the basic region of the c-Jun DNA-binding domain is essential for repression by E1A .
	manualset3
198167	6	416230	7	NULL	NULL	0	NULL	c-Jun DNA-binding domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using chimeras of c-Jun and EB1 , we demonstrate that a 12 amino acid region in the basic region of the c-Jun DNA-binding domain is essential for repression by E1A .
	manualset3
198168	7	416230	7	NULL	NULL	0	NULL	repression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using chimeras of c-Jun and EB1 , we demonstrate that a 12 amino acid region in the basic region of the c-Jun DNA-binding domain is essential for repression by E1A .
	manualset3
198169	8	416230	7	NULL	NULL	0	NULL	E1A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using chimeras of c-Jun and EB1 , we demonstrate that a 12 amino acid region in the basic region of the c-Jun DNA-binding domain is essential for repression by E1A .
	manualset3
198171	1	416231	7	NULL	NULL	NULL	NULL	 treatment 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After treatment with methyl jasmonate ( MJ ) we investigated the expression of all isoprenyl diphosphate synthase genes characterized to date from Norway spruce and correlated this with formation of traumatic resin ducts and terpene accumulation .
	manualset3
198172	2	416231	7	NULL	NULL	0	NULL	methyl jasmonate ( MJ )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment with methyl jasmonate ( MJ ) we investigated the expression of all isoprenyl diphosphate synthase genes characterized to date from Norway spruce and correlated this with formation of traumatic resin ducts and terpene accumulation .
	manualset3
198173	3	416231	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment with methyl jasmonate ( MJ ) we investigated the expression of all isoprenyl diphosphate synthase genes characterized to date from Norway spruce and correlated this with formation of traumatic resin ducts and terpene accumulation .
	manualset3
198174	4	416231	7	NULL	NULL	0	NULL	isoprenyl diphosphate synthase genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment with methyl jasmonate ( MJ ) we investigated the expression of all isoprenyl diphosphate synthase genes characterized to date from Norway spruce and correlated this with formation of traumatic resin ducts and terpene accumulation .
	manualset3
198175	5	416231	7	NULL	NULL	0	NULL	date	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment with methyl jasmonate ( MJ ) we investigated the expression of all isoprenyl diphosphate synthase genes characterized to date from Norway spruce and correlated this with formation of traumatic resin ducts and terpene accumulation .
	manualset3
198176	6	416231	7	NULL	NULL	0	NULL	Norway spruce	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment with methyl jasmonate ( MJ ) we investigated the expression of all isoprenyl diphosphate synthase genes characterized to date from Norway spruce and correlated this with formation of traumatic resin ducts and terpene accumulation .
	manualset3
198177	7	416231	7	NULL	NULL	NULL	NULL	formation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After treatment with methyl jasmonate ( MJ ) we investigated the expression of all isoprenyl diphosphate synthase genes characterized to date from Norway spruce and correlated this with formation of traumatic resin ducts and terpene accumulation .
	manualset3
198178	8	416231	7	NULL	NULL	0	NULL	 traumatic resin ducts 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment with methyl jasmonate ( MJ ) we investigated the expression of all isoprenyl diphosphate synthase genes characterized to date from Norway spruce and correlated this with formation of traumatic resin ducts and terpene accumulation .
	manualset3
198179	9	416231	7	NULL	NULL	NULL	NULL	terpene accumulation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After treatment with methyl jasmonate ( MJ ) we investigated the expression of all isoprenyl diphosphate synthase genes characterized to date from Norway spruce and correlated this with formation of traumatic resin ducts and terpene accumulation .
	manualset3
198180	1	416232	7	NULL	NULL	0	NULL	confocal microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using confocal microscopy of live PC12 cells , transiently transfected with a chimera of green fluorescent protein ( GFP ) fused to the N-terminus of centaurin-alpha1 ( GFP-centaurin-alpha1 ) , we demonstrated the rapid plasma membrane recruitment of cytosolic GFP-centaurin-alpha1 following stimulation with either nerve growth factor or epidermal growth factor .
	manualset3
198181	2	416232	7	NULL	NULL	0	NULL	live PC12 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using confocal microscopy of live PC12 cells , transiently transfected with a chimera of green fluorescent protein ( GFP ) fused to the N-terminus of centaurin-alpha1 ( GFP-centaurin-alpha1 ) , we demonstrated the rapid plasma membrane recruitment of cytosolic GFP-centaurin-alpha1 following stimulation with either nerve growth factor or epidermal growth factor .
	manualset3
198182	3	416232	7	NULL	NULL	0	NULL	chimera	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using confocal microscopy of live PC12 cells , transiently transfected with a chimera of green fluorescent protein ( GFP ) fused to the N-terminus of centaurin-alpha1 ( GFP-centaurin-alpha1 ) , we demonstrated the rapid plasma membrane recruitment of cytosolic GFP-centaurin-alpha1 following stimulation with either nerve growth factor or epidermal growth factor .
	manualset3
198183	4	416232	7	NULL	NULL	0	NULL	 green fluorescent protein ( GFP ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using confocal microscopy of live PC12 cells , transiently transfected with a chimera of green fluorescent protein ( GFP ) fused to the N-terminus of centaurin-alpha1 ( GFP-centaurin-alpha1 ) , we demonstrated the rapid plasma membrane recruitment of cytosolic GFP-centaurin-alpha1 following stimulation with either nerve growth factor or epidermal growth factor .
	manualset3
198184	5	416232	7	NULL	NULL	0	NULL	N-terminus 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using confocal microscopy of live PC12 cells , transiently transfected with a chimera of green fluorescent protein ( GFP ) fused to the N-terminus of centaurin-alpha1 ( GFP-centaurin-alpha1 ) , we demonstrated the rapid plasma membrane recruitment of cytosolic GFP-centaurin-alpha1 following stimulation with either nerve growth factor or epidermal growth factor .
	manualset3
198185	6	416232	7	NULL	NULL	0	NULL	centaurin-alpha1 ( GFP-centaurin-alpha1 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using confocal microscopy of live PC12 cells , transiently transfected with a chimera of green fluorescent protein ( GFP ) fused to the N-terminus of centaurin-alpha1 ( GFP-centaurin-alpha1 ) , we demonstrated the rapid plasma membrane recruitment of cytosolic GFP-centaurin-alpha1 following stimulation with either nerve growth factor or epidermal growth factor .
	manualset3
198186	7	416232	7	NULL	NULL	0	NULL	rapid plasma membrane recruitment	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using confocal microscopy of live PC12 cells , transiently transfected with a chimera of green fluorescent protein ( GFP ) fused to the N-terminus of centaurin-alpha1 ( GFP-centaurin-alpha1 ) , we demonstrated the rapid plasma membrane recruitment of cytosolic GFP-centaurin-alpha1 following stimulation with either nerve growth factor or epidermal growth factor .
	manualset3
198187	8	416232	7	NULL	NULL	0	NULL	cytosolic GFP-centaurin-alpha1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using confocal microscopy of live PC12 cells , transiently transfected with a chimera of green fluorescent protein ( GFP ) fused to the N-terminus of centaurin-alpha1 ( GFP-centaurin-alpha1 ) , we demonstrated the rapid plasma membrane recruitment of cytosolic GFP-centaurin-alpha1 following stimulation with either nerve growth factor or epidermal growth factor .
	manualset3
198188	9	416232	7	NULL	NULL	0	NULL	stimulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using confocal microscopy of live PC12 cells , transiently transfected with a chimera of green fluorescent protein ( GFP ) fused to the N-terminus of centaurin-alpha1 ( GFP-centaurin-alpha1 ) , we demonstrated the rapid plasma membrane recruitment of cytosolic GFP-centaurin-alpha1 following stimulation with either nerve growth factor or epidermal growth factor .
	manualset3
198189	10	416232	7	NULL	NULL	0	NULL	nerve growth factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using confocal microscopy of live PC12 cells , transiently transfected with a chimera of green fluorescent protein ( GFP ) fused to the N-terminus of centaurin-alpha1 ( GFP-centaurin-alpha1 ) , we demonstrated the rapid plasma membrane recruitment of cytosolic GFP-centaurin-alpha1 following stimulation with either nerve growth factor or epidermal growth factor .
	manualset3
198190	11	416232	7	NULL	NULL	0	NULL	 epidermal growth factor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using confocal microscopy of live PC12 cells , transiently transfected with a chimera of green fluorescent protein ( GFP ) fused to the N-terminus of centaurin-alpha1 ( GFP-centaurin-alpha1 ) , we demonstrated the rapid plasma membrane recruitment of cytosolic GFP-centaurin-alpha1 following stimulation with either nerve growth factor or epidermal growth factor .
	manualset3
198191	1	416233	7	NULL	NULL	0	NULL	cross-sectional survey data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Using cross-sectional survey data from a representative sample of married Egyptian women ( N = 5 , 240 ) , associations between forced intercourse and husband 's control , as well as other relevant sociodemographic factors , were assessed through binary logistic regression models .
	manualset3
198192	2	416233	7	NULL	NULL	0	NULL	 representative sample	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using cross-sectional survey data from a representative sample of married Egyptian women ( N = 5 , 240 ) , associations between forced intercourse and husband 's control , as well as other relevant sociodemographic factors , were assessed through binary logistic regression models .
	manualset3
198193	3	416233	7	NULL	NULL	0	NULL	married Egyptian women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using cross-sectional survey data from a representative sample of married Egyptian women ( N = 5 , 240 ) , associations between forced intercourse and husband 's control , as well as other relevant sociodemographic factors , were assessed through binary logistic regression models .
	manualset3
198194	4	416233	7	NULL	NULL	0	NULL	N = 5 , 240	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Using cross-sectional survey data from a representative sample of married Egyptian women ( N = 5 , 240 ) , associations between forced intercourse and husband 's control , as well as other relevant sociodemographic factors , were assessed through binary logistic regression models .
	manualset3
198195	5	416233	7	NULL	NULL	0	NULL	 associations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Using cross-sectional survey data from a representative sample of married Egyptian women ( N = 5 , 240 ) , associations between forced intercourse and husband 's control , as well as other relevant sociodemographic factors , were assessed through binary logistic regression models .
	manualset3
198196	6	416233	7	NULL	NULL	0	NULL	forced intercourse	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using cross-sectional survey data from a representative sample of married Egyptian women ( N = 5 , 240 ) , associations between forced intercourse and husband 's control , as well as other relevant sociodemographic factors , were assessed through binary logistic regression models .
	manualset3
198197	7	416233	7	NULL	NULL	0	NULL	husband 's control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using cross-sectional survey data from a representative sample of married Egyptian women ( N = 5 , 240 ) , associations between forced intercourse and husband 's control , as well as other relevant sociodemographic factors , were assessed through binary logistic regression models .
	manualset3
198198	8	416233	7	NULL	NULL	0	NULL	sociodemographic factors	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Using cross-sectional survey data from a representative sample of married Egyptian women ( N = 5 , 240 ) , associations between forced intercourse and husband 's control , as well as other relevant sociodemographic factors , were assessed through binary logistic regression models .
	manualset3
198199	9	416233	7	NULL	NULL	0	NULL	binary logistic regression models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Using cross-sectional survey data from a representative sample of married Egyptian women ( N = 5 , 240 ) , associations between forced intercourse and husband 's control , as well as other relevant sociodemographic factors , were assessed through binary logistic regression models .
	manualset3
198200	1	416234	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Using data from a set of cell migration experiments reported in the literature , we show how to determine the value of the random motility coefficient and its dependence upon concentration of a tripeptide chemotactic attractant , as well as the value of the chemotaxis coefficient , assumed here to be independent of attractant concentration .
	manualset3
198201	2	416234	7	NULL	NULL	0	NULL	set	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using data from a set of cell migration experiments reported in the literature , we show how to determine the value of the random motility coefficient and its dependence upon concentration of a tripeptide chemotactic attractant , as well as the value of the chemotaxis coefficient , assumed here to be independent of attractant concentration .
	manualset3
198202	3	416234	7	NULL	NULL	0	NULL	cell migration experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using data from a set of cell migration experiments reported in the literature , we show how to determine the value of the random motility coefficient and its dependence upon concentration of a tripeptide chemotactic attractant , as well as the value of the chemotaxis coefficient , assumed here to be independent of attractant concentration .
	manualset3
198203	4	416234	7	NULL	NULL	0	NULL	 literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Using data from a set of cell migration experiments reported in the literature , we show how to determine the value of the random motility coefficient and its dependence upon concentration of a tripeptide chemotactic attractant , as well as the value of the chemotaxis coefficient , assumed here to be independent of attractant concentration .
	manualset3
198204	5	416234	7	NULL	NULL	0	NULL	 value 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using data from a set of cell migration experiments reported in the literature , we show how to determine the value of the random motility coefficient and its dependence upon concentration of a tripeptide chemotactic attractant , as well as the value of the chemotaxis coefficient , assumed here to be independent of attractant concentration .
	manualset3
198205	6	416234	7	NULL	NULL	0	NULL	random motility coefficient 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Using data from a set of cell migration experiments reported in the literature , we show how to determine the value of the random motility coefficient and its dependence upon concentration of a tripeptide chemotactic attractant , as well as the value of the chemotaxis coefficient , assumed here to be independent of attractant concentration .
	manualset3
198206	7	416234	7	NULL	NULL	0	NULL	concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using data from a set of cell migration experiments reported in the literature , we show how to determine the value of the random motility coefficient and its dependence upon concentration of a tripeptide chemotactic attractant , as well as the value of the chemotaxis coefficient , assumed here to be independent of attractant concentration .
	manualset3
198207	8	416234	7	NULL	NULL	0	NULL	tripeptide chemotactic attractant	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Using data from a set of cell migration experiments reported in the literature , we show how to determine the value of the random motility coefficient and its dependence upon concentration of a tripeptide chemotactic attractant , as well as the value of the chemotaxis coefficient , assumed here to be independent of attractant concentration .
	manualset3
198208	9	416234	7	NULL	NULL	0	NULL	value 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using data from a set of cell migration experiments reported in the literature , we show how to determine the value of the random motility coefficient and its dependence upon concentration of a tripeptide chemotactic attractant , as well as the value of the chemotaxis coefficient , assumed here to be independent of attractant concentration .
	manualset3
198209	10	416234	7	NULL	NULL	0	NULL	chemotaxis coefficient	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Using data from a set of cell migration experiments reported in the literature , we show how to determine the value of the random motility coefficient and its dependence upon concentration of a tripeptide chemotactic attractant , as well as the value of the chemotaxis coefficient , assumed here to be independent of attractant concentration .
	manualset3
198210	11	416234	7	NULL	NULL	0	NULL	attractant concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using data from a set of cell migration experiments reported in the literature , we show how to determine the value of the random motility coefficient and its dependence upon concentration of a tripeptide chemotactic attractant , as well as the value of the chemotaxis coefficient , assumed here to be independent of attractant concentration .
	manualset3
198211	1	416235	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Using data from patients accrued after randomization to the control group , we fail to find evidence that either chemotherapy alone or chemoimmunotherapy improves OS or RFS when contrasted to outcomes obtained by patients on the control arm .
	manualset3
198212	2	416235	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using data from patients accrued after randomization to the control group , we fail to find evidence that either chemotherapy alone or chemoimmunotherapy improves OS or RFS when contrasted to outcomes obtained by patients on the control arm .
	manualset3
198213	3	416235	7	NULL	NULL	0	NULL	randomization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using data from patients accrued after randomization to the control group , we fail to find evidence that either chemotherapy alone or chemoimmunotherapy improves OS or RFS when contrasted to outcomes obtained by patients on the control arm .
	manualset3
198214	4	416235	7	NULL	NULL	0	NULL	control group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using data from patients accrued after randomization to the control group , we fail to find evidence that either chemotherapy alone or chemoimmunotherapy improves OS or RFS when contrasted to outcomes obtained by patients on the control arm .
	manualset3
198215	5	416235	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using data from patients accrued after randomization to the control group , we fail to find evidence that either chemotherapy alone or chemoimmunotherapy improves OS or RFS when contrasted to outcomes obtained by patients on the control arm .
	manualset3
198216	6	416235	7	NULL	NULL	0	NULL	chemotherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Using data from patients accrued after randomization to the control group , we fail to find evidence that either chemotherapy alone or chemoimmunotherapy improves OS or RFS when contrasted to outcomes obtained by patients on the control arm .
	manualset3
198217	7	416235	7	NULL	NULL	0	NULL	chemoimmunotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Using data from patients accrued after randomization to the control group , we fail to find evidence that either chemotherapy alone or chemoimmunotherapy improves OS or RFS when contrasted to outcomes obtained by patients on the control arm .
	manualset3
198218	8	416235	7	NULL	NULL	0	NULL	OS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using data from patients accrued after randomization to the control group , we fail to find evidence that either chemotherapy alone or chemoimmunotherapy improves OS or RFS when contrasted to outcomes obtained by patients on the control arm .
	manualset3
198219	9	416235	7	NULL	NULL	0	NULL	RFS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using data from patients accrued after randomization to the control group , we fail to find evidence that either chemotherapy alone or chemoimmunotherapy improves OS or RFS when contrasted to outcomes obtained by patients on the control arm .
	manualset3
198220	10	416235	7	NULL	NULL	0	NULL	outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using data from patients accrued after randomization to the control group , we fail to find evidence that either chemotherapy alone or chemoimmunotherapy improves OS or RFS when contrasted to outcomes obtained by patients on the control arm .
	manualset3
198221	11	416235	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using data from patients accrued after randomization to the control group , we fail to find evidence that either chemotherapy alone or chemoimmunotherapy improves OS or RFS when contrasted to outcomes obtained by patients on the control arm .
	manualset3
198222	12	416235	7	NULL	NULL	0	NULL	control arm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using data from patients accrued after randomization to the control group , we fail to find evidence that either chemotherapy alone or chemoimmunotherapy improves OS or RFS when contrasted to outcomes obtained by patients on the control arm .
	manualset3
198223	1	416236	7	NULL	NULL	0	NULL	H2O2-Fe treated nuclei	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using either H2O2-Fe treated nuclei or As2O3-treated cells , digestion with either NE or EnIII + Fpg generated the same amount of breaks , and subsequent treatment with EnIII + Fpg resulted in no increase in breaks in NE-digested cells and vice versa .
	manualset3
198224	2	416236	7	NULL	NULL	0	NULL	As2O3-treated cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using either H2O2-Fe treated nuclei or As2O3-treated cells , digestion with either NE or EnIII + Fpg generated the same amount of breaks , and subsequent treatment with EnIII + Fpg resulted in no increase in breaks in NE-digested cells and vice versa .
	manualset3
198225	3	416236	7	NULL	NULL	0	NULL	digestion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using either H2O2-Fe treated nuclei or As2O3-treated cells , digestion with either NE or EnIII + Fpg generated the same amount of breaks , and subsequent treatment with EnIII + Fpg resulted in no increase in breaks in NE-digested cells and vice versa .
	manualset3
198226	4	416236	7	NULL	NULL	0	NULL	NE	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Using either H2O2-Fe treated nuclei or As2O3-treated cells , digestion with either NE or EnIII + Fpg generated the same amount of breaks , and subsequent treatment with EnIII + Fpg resulted in no increase in breaks in NE-digested cells and vice versa .
	manualset3
198227	5	416236	7	NULL	NULL	0	NULL	EnIII + Fpg	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using either H2O2-Fe treated nuclei or As2O3-treated cells , digestion with either NE or EnIII + Fpg generated the same amount of breaks , and subsequent treatment with EnIII + Fpg resulted in no increase in breaks in NE-digested cells and vice versa .
	manualset3
198228	6	416236	7	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using either H2O2-Fe treated nuclei or As2O3-treated cells , digestion with either NE or EnIII + Fpg generated the same amount of breaks , and subsequent treatment with EnIII + Fpg resulted in no increase in breaks in NE-digested cells and vice versa .
	manualset3
198229	7	416236	7	NULL	NULL	0	NULL	 breaks	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using either H2O2-Fe treated nuclei or As2O3-treated cells , digestion with either NE or EnIII + Fpg generated the same amount of breaks , and subsequent treatment with EnIII + Fpg resulted in no increase in breaks in NE-digested cells and vice versa .
	manualset3
198230	8	416236	7	NULL	NULL	0	NULL	treatment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using either H2O2-Fe treated nuclei or As2O3-treated cells , digestion with either NE or EnIII + Fpg generated the same amount of breaks , and subsequent treatment with EnIII + Fpg resulted in no increase in breaks in NE-digested cells and vice versa .
	manualset3
198231	9	416236	7	NULL	NULL	0	NULL	EnIII + Fpg 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using either H2O2-Fe treated nuclei or As2O3-treated cells , digestion with either NE or EnIII + Fpg generated the same amount of breaks , and subsequent treatment with EnIII + Fpg resulted in no increase in breaks in NE-digested cells and vice versa .
	manualset3
198232	10	416236	7	NULL	NULL	0	NULL	no increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using either H2O2-Fe treated nuclei or As2O3-treated cells , digestion with either NE or EnIII + Fpg generated the same amount of breaks , and subsequent treatment with EnIII + Fpg resulted in no increase in breaks in NE-digested cells and vice versa .
	manualset3
198233	11	416236	7	NULL	NULL	0	NULL	breaks	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using either H2O2-Fe treated nuclei or As2O3-treated cells , digestion with either NE or EnIII + Fpg generated the same amount of breaks , and subsequent treatment with EnIII + Fpg resulted in no increase in breaks in NE-digested cells and vice versa .
	manualset3
198234	12	416236	7	NULL	NULL	0	NULL	NE-digested cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using either H2O2-Fe treated nuclei or As2O3-treated cells , digestion with either NE or EnIII + Fpg generated the same amount of breaks , and subsequent treatment with EnIII + Fpg resulted in no increase in breaks in NE-digested cells and vice versa .
	manualset3
198235	1	416237	7	NULL	NULL	0	NULL	epsilon-peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Using epsilon-peptide as the substrate , the first peak of activity was dependent upon Ca2 + and 4beta-PDBu ( PDBu = phorbol 12 , 13-dibutyrate ) , and represented a mixture of PKCs alpha , betaI and betaII .
	manualset3
198236	2	416237	7	NULL	NULL	0	NULL	substrate	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Using epsilon-peptide as the substrate , the first peak of activity was dependent upon Ca2 + and 4beta-PDBu ( PDBu = phorbol 12 , 13-dibutyrate ) , and represented a mixture of PKCs alpha , betaI and betaII .
	manualset3
198237	3	416237	7	NULL	NULL	0	NULL	first peak of activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using epsilon-peptide as the substrate , the first peak of activity was dependent upon Ca2 + and 4beta-PDBu ( PDBu = phorbol 12 , 13-dibutyrate ) , and represented a mixture of PKCs alpha , betaI and betaII .
	manualset3
198238	4	416237	7	NULL	NULL	0	NULL	Ca2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Using epsilon-peptide as the substrate , the first peak of activity was dependent upon Ca2 + and 4beta-PDBu ( PDBu = phorbol 12 , 13-dibutyrate ) , and represented a mixture of PKCs alpha , betaI and betaII .
	manualset3
198239	5	416237	7	NULL	NULL	0	NULL	4beta-PDBu ( PDBu = phorbol 12 , 13-dibutyrate )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using epsilon-peptide as the substrate , the first peak of activity was dependent upon Ca2 + and 4beta-PDBu ( PDBu = phorbol 12 , 13-dibutyrate ) , and represented a mixture of PKCs alpha , betaI and betaII .
	manualset3
198240	6	416237	7	NULL	NULL	0	NULL	mixture	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using epsilon-peptide as the substrate , the first peak of activity was dependent upon Ca2 + and 4beta-PDBu ( PDBu = phorbol 12 , 13-dibutyrate ) , and represented a mixture of PKCs alpha , betaI and betaII .
	manualset3
198241	7	416237	7	NULL	NULL	0	NULL	PKCs alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using epsilon-peptide as the substrate , the first peak of activity was dependent upon Ca2 + and 4beta-PDBu ( PDBu = phorbol 12 , 13-dibutyrate ) , and represented a mixture of PKCs alpha , betaI and betaII .
	manualset3
198242	8	416237	7	NULL	NULL	0	NULL	PKCs betaI	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using epsilon-peptide as the substrate , the first peak of activity was dependent upon Ca2 + and 4beta-PDBu ( PDBu = phorbol 12 , 13-dibutyrate ) , and represented a mixture of PKCs alpha , betaI and betaII .
	manualset3
198243	9	416237	7	NULL	NULL	0	NULL	PKCbetaII	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using epsilon-peptide as the substrate , the first peak of activity was dependent upon Ca2 + and 4beta-PDBu ( PDBu = phorbol 12 , 13-dibutyrate ) , and represented a mixture of PKCs alpha , betaI and betaII .
	manualset3
198244	1	416238	7	NULL	NULL	0	NULL	estrogen receptor ( ER ) alpha knockout mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Using estrogen receptor ( ER ) alpha and beta knockout mice and wild-type littermates , we investigated the role of ERs in estradiol effects on multiple pathways important for hippocampal plasticity and learning .
	manualset3
198245	2	416238	7	NULL	NULL	0	NULL	estrogen receptor ( ER ) beta knockout mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Using estrogen receptor ( ER ) alpha and beta knockout mice and wild-type littermates , we investigated the role of ERs in estradiol effects on multiple pathways important for hippocampal plasticity and learning .
	manualset3
198246	3	416238	7	NULL	NULL	0	NULL	wild-type littermates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Using estrogen receptor ( ER ) alpha and beta knockout mice and wild-type littermates , we investigated the role of ERs in estradiol effects on multiple pathways important for hippocampal plasticity and learning .
	manualset3
198247	4	416238	7	NULL	NULL	0	NULL	 role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using estrogen receptor ( ER ) alpha and beta knockout mice and wild-type littermates , we investigated the role of ERs in estradiol effects on multiple pathways important for hippocampal plasticity and learning .
	manualset3
198248	5	416238	7	NULL	NULL	0	NULL	ERs	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using estrogen receptor ( ER ) alpha and beta knockout mice and wild-type littermates , we investigated the role of ERs in estradiol effects on multiple pathways important for hippocampal plasticity and learning .
	manualset3
198249	6	416238	7	NULL	NULL	0	NULL	estradiol effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using estrogen receptor ( ER ) alpha and beta knockout mice and wild-type littermates , we investigated the role of ERs in estradiol effects on multiple pathways important for hippocampal plasticity and learning .
	manualset3
198250	7	416238	7	NULL	NULL	NULL	NULL	multiple pathways	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using estrogen receptor ( ER ) alpha and beta knockout mice and wild-type littermates , we investigated the role of ERs in estradiol effects on multiple pathways important for hippocampal plasticity and learning .
	manualset3
198251	8	416238	7	NULL	NULL	0	NULL	hippocampal plasticity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using estrogen receptor ( ER ) alpha and beta knockout mice and wild-type littermates , we investigated the role of ERs in estradiol effects on multiple pathways important for hippocampal plasticity and learning .
	manualset3
198252	9	416238	7	NULL	NULL	0	NULL	learning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using estrogen receptor ( ER ) alpha and beta knockout mice and wild-type littermates , we investigated the role of ERs in estradiol effects on multiple pathways important for hippocampal plasticity and learning .
	manualset3
198253	1	416239	7	NULL	NULL	0	NULL	treatment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment with phorbol esters , a high percentage of cells from these three lines synthesize keratin IF identified by immunoblotting as keratin 8 and 18 polypeptides , which are expressed by single epithelia and epithelial cells in early embryonic development .
	manualset3
198254	2	416239	7	NULL	NULL	0	NULL	phorbol esters	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment with phorbol esters , a high percentage of cells from these three lines synthesize keratin IF identified by immunoblotting as keratin 8 and 18 polypeptides , which are expressed by single epithelia and epithelial cells in early embryonic development .
	manualset3
198255	3	416239	7	NULL	NULL	0	NULL	high percentage 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment with phorbol esters , a high percentage of cells from these three lines synthesize keratin IF identified by immunoblotting as keratin 8 and 18 polypeptides , which are expressed by single epithelia and epithelial cells in early embryonic development .
	manualset3
198256	4	416239	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment with phorbol esters , a high percentage of cells from these three lines synthesize keratin IF identified by immunoblotting as keratin 8 and 18 polypeptides , which are expressed by single epithelia and epithelial cells in early embryonic development .
	manualset3
198257	5	416239	7	NULL	NULL	0	NULL	 three lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment with phorbol esters , a high percentage of cells from these three lines synthesize keratin IF identified by immunoblotting as keratin 8 and 18 polypeptides , which are expressed by single epithelia and epithelial cells in early embryonic development .
	manualset3
198258	6	416239	7	NULL	NULL	0	NULL	keratin IF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment with phorbol esters , a high percentage of cells from these three lines synthesize keratin IF identified by immunoblotting as keratin 8 and 18 polypeptides , which are expressed by single epithelia and epithelial cells in early embryonic development .
	manualset3
198259	7	416239	7	NULL	NULL	0	NULL	immunoblotting	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment with phorbol esters , a high percentage of cells from these three lines synthesize keratin IF identified by immunoblotting as keratin 8 and 18 polypeptides , which are expressed by single epithelia and epithelial cells in early embryonic development .
	manualset3
198260	8	416239	7	NULL	NULL	NULL	NULL	keratin 8	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After treatment with phorbol esters , a high percentage of cells from these three lines synthesize keratin IF identified by immunoblotting as keratin 8 and 18 polypeptides , which are expressed by single epithelia and epithelial cells in early embryonic development .
	manualset3
198261	9	416239	7	NULL	NULL	0	NULL	18 polypeptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment with phorbol esters , a high percentage of cells from these three lines synthesize keratin IF identified by immunoblotting as keratin 8 and 18 polypeptides , which are expressed by single epithelia and epithelial cells in early embryonic development .
	manualset3
198262	10	416239	7	NULL	NULL	0	NULL	single epithelia cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment with phorbol esters , a high percentage of cells from these three lines synthesize keratin IF identified by immunoblotting as keratin 8 and 18 polypeptides , which are expressed by single epithelia and epithelial cells in early embryonic development .
	manualset3
198263	11	416239	7	NULL	NULL	0	NULL	epithelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment with phorbol esters , a high percentage of cells from these three lines synthesize keratin IF identified by immunoblotting as keratin 8 and 18 polypeptides , which are expressed by single epithelia and epithelial cells in early embryonic development .
	manualset3
198264	12	416239	7	NULL	NULL	0	NULL	early embryonic development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After treatment with phorbol esters , a high percentage of cells from these three lines synthesize keratin IF identified by immunoblotting as keratin 8 and 18 polypeptides , which are expressed by single epithelia and epithelial cells in early embryonic development .
	manualset3
198265	1	416240	7	NULL	NULL	0	NULL	fish crows ( Corvus ossifragus )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Using fish crows ( Corvus ossifragus ) as a model , we found that none of eight crows that received two high doses of vaccine ( approximately 100 , 000 plaque-forming units ( PFU ) ) developed viremia and only one developed WNV-neutralizing antibodies .
	manualset3
198266	2	416240	7	NULL	NULL	0	NULL	model	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Using fish crows ( Corvus ossifragus ) as a model , we found that none of eight crows that received two high doses of vaccine ( approximately 100 , 000 plaque-forming units ( PFU ) ) developed viremia and only one developed WNV-neutralizing antibodies .
	manualset3
198267	3	416240	7	NULL	NULL	0	NULL	eight crows	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Using fish crows ( Corvus ossifragus ) as a model , we found that none of eight crows that received two high doses of vaccine ( approximately 100 , 000 plaque-forming units ( PFU ) ) developed viremia and only one developed WNV-neutralizing antibodies .
	manualset3
198268	4	416240	7	NULL	NULL	0	NULL	two high doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using fish crows ( Corvus ossifragus ) as a model , we found that none of eight crows that received two high doses of vaccine ( approximately 100 , 000 plaque-forming units ( PFU ) ) developed viremia and only one developed WNV-neutralizing antibodies .
	manualset3
198269	5	416240	7	NULL	NULL	0	NULL	vaccine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Using fish crows ( Corvus ossifragus ) as a model , we found that none of eight crows that received two high doses of vaccine ( approximately 100 , 000 plaque-forming units ( PFU ) ) developed viremia and only one developed WNV-neutralizing antibodies .
	manualset3
198270	6	416240	7	NULL	NULL	0	NULL	 100 , 000 plaque-forming units ( PFU )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using fish crows ( Corvus ossifragus ) as a model , we found that none of eight crows that received two high doses of vaccine ( approximately 100 , 000 plaque-forming units ( PFU ) ) developed viremia and only one developed WNV-neutralizing antibodies .
	manualset3
198271	7	416240	7	NULL	NULL	0	NULL	viremia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using fish crows ( Corvus ossifragus ) as a model , we found that none of eight crows that received two high doses of vaccine ( approximately 100 , 000 plaque-forming units ( PFU ) ) developed viremia and only one developed WNV-neutralizing antibodies .
	manualset3
198272	8	416240	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using fish crows ( Corvus ossifragus ) as a model , we found that none of eight crows that received two high doses of vaccine ( approximately 100 , 000 plaque-forming units ( PFU ) ) developed viremia and only one developed WNV-neutralizing antibodies .
	manualset3
198273	9	416240	7	NULL	NULL	0	NULL	WNV-neutralizing antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using fish crows ( Corvus ossifragus ) as a model , we found that none of eight crows that received two high doses of vaccine ( approximately 100 , 000 plaque-forming units ( PFU ) ) developed viremia and only one developed WNV-neutralizing antibodies .
	manualset3
198274	1	416241	7	NULL	NULL	0	NULL	fluorescence-activated cell sorting ( FACS )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using fluorescence-activated cell sorting ( FACS ) , human marrow cells were fractionated into Hermeshi , Hermesmed , and Hermeslo populations according to the expression of both the Hermes-1 and Hermes-3 epitopes .
	manualset3
198275	2	416241	7	NULL	NULL	0	NULL	human marrow cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using fluorescence-activated cell sorting ( FACS ) , human marrow cells were fractionated into Hermeshi , Hermesmed , and Hermeslo populations according to the expression of both the Hermes-1 and Hermes-3 epitopes .
	manualset3
198276	3	416241	7	NULL	NULL	0	NULL	Hermeshi population	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using fluorescence-activated cell sorting ( FACS ) , human marrow cells were fractionated into Hermeshi , Hermesmed , and Hermeslo populations according to the expression of both the Hermes-1 and Hermes-3 epitopes .
	manualset3
198277	4	416241	7	NULL	NULL	0	NULL	Hermesmed population	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using fluorescence-activated cell sorting ( FACS ) , human marrow cells were fractionated into Hermeshi , Hermesmed , and Hermeslo populations according to the expression of both the Hermes-1 and Hermes-3 epitopes .
	manualset3
198278	5	416241	7	NULL	NULL	0	NULL	Hermeslo populations	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using fluorescence-activated cell sorting ( FACS ) , human marrow cells were fractionated into Hermeshi , Hermesmed , and Hermeslo populations according to the expression of both the Hermes-1 and Hermes-3 epitopes .
	manualset3
198279	6	416241	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using fluorescence-activated cell sorting ( FACS ) , human marrow cells were fractionated into Hermeshi , Hermesmed , and Hermeslo populations according to the expression of both the Hermes-1 and Hermes-3 epitopes .
	manualset3
198280	7	416241	7	NULL	NULL	0	NULL	Hermes-1 epitope	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using fluorescence-activated cell sorting ( FACS ) , human marrow cells were fractionated into Hermeshi , Hermesmed , and Hermeslo populations according to the expression of both the Hermes-1 and Hermes-3 epitopes .
	manualset3
198281	8	416241	7	NULL	NULL	0	NULL	 Hermes-3 epitopes	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using fluorescence-activated cell sorting ( FACS ) , human marrow cells were fractionated into Hermeshi , Hermesmed , and Hermeslo populations according to the expression of both the Hermes-1 and Hermes-3 epitopes .
	manualset3
198282	1	416242	7	NULL	NULL	0	NULL	 fluorescence microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using fluorescence microscopy , we investigated assembly at the AWI of a model protein , human serum albumin minimally labeled with Texas Red fluorophore .
	manualset3
198283	2	416242	7	NULL	NULL	0	NULL	assembly	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using fluorescence microscopy , we investigated assembly at the AWI of a model protein , human serum albumin minimally labeled with Texas Red fluorophore .
	manualset3
198284	3	416242	7	NULL	NULL	0	NULL	AWI	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using fluorescence microscopy , we investigated assembly at the AWI of a model protein , human serum albumin minimally labeled with Texas Red fluorophore .
	manualset3
198285	4	416242	7	NULL	NULL	0	NULL	model protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using fluorescence microscopy , we investigated assembly at the AWI of a model protein , human serum albumin minimally labeled with Texas Red fluorophore .
	manualset3
198286	5	416242	7	NULL	NULL	0	NULL	human serum albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using fluorescence microscopy , we investigated assembly at the AWI of a model protein , human serum albumin minimally labeled with Texas Red fluorophore .
	manualset3
198287	6	416242	7	NULL	NULL	0	NULL	Texas Red fluorophore 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using fluorescence microscopy , we investigated assembly at the AWI of a model protein , human serum albumin minimally labeled with Texas Red fluorophore .
	manualset3
198288	1	416243	7	NULL	NULL	0	NULL	high-performance liquid chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using high-performance liquid chromatography to isolate inhibitin , culture media from HL60 and H. Ep2 cells were identically treated , and inhibitin isolated from H. Ep2 cells had the same retention time as that shown by promyelocyte inhibitin .
	manualset3
198289	2	416243	7	NULL	NULL	0	NULL	 inhibitin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using high-performance liquid chromatography to isolate inhibitin , culture media from HL60 and H. Ep2 cells were identically treated , and inhibitin isolated from H. Ep2 cells had the same retention time as that shown by promyelocyte inhibitin .
	manualset3
198290	3	416243	7	NULL	NULL	0	NULL	 culture media	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using high-performance liquid chromatography to isolate inhibitin , culture media from HL60 and H. Ep2 cells were identically treated , and inhibitin isolated from H. Ep2 cells had the same retention time as that shown by promyelocyte inhibitin .
	manualset3
198291	4	416243	7	NULL	NULL	0	NULL	HL60 cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using high-performance liquid chromatography to isolate inhibitin , culture media from HL60 and H. Ep2 cells were identically treated , and inhibitin isolated from H. Ep2 cells had the same retention time as that shown by promyelocyte inhibitin .
	manualset3
198292	5	416243	7	NULL	NULL	0	NULL	H. Ep2 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using high-performance liquid chromatography to isolate inhibitin , culture media from HL60 and H. Ep2 cells were identically treated , and inhibitin isolated from H. Ep2 cells had the same retention time as that shown by promyelocyte inhibitin .
	manualset3
198293	6	416243	7	NULL	NULL	0	NULL	 inhibitin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using high-performance liquid chromatography to isolate inhibitin , culture media from HL60 and H. Ep2 cells were identically treated , and inhibitin isolated from H. Ep2 cells had the same retention time as that shown by promyelocyte inhibitin .
	manualset3
198294	7	416243	7	NULL	NULL	0	NULL	H. Ep2 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using high-performance liquid chromatography to isolate inhibitin , culture media from HL60 and H. Ep2 cells were identically treated , and inhibitin isolated from H. Ep2 cells had the same retention time as that shown by promyelocyte inhibitin .
	manualset3
198295	8	416243	7	NULL	NULL	0	NULL	retention time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Using high-performance liquid chromatography to isolate inhibitin , culture media from HL60 and H. Ep2 cells were identically treated , and inhibitin isolated from H. Ep2 cells had the same retention time as that shown by promyelocyte inhibitin .
	manualset3
198296	9	416243	7	NULL	NULL	0	NULL	promyelocyte inhibitin 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using high-performance liquid chromatography to isolate inhibitin , culture media from HL60 and H. Ep2 cells were identically treated , and inhibitin isolated from H. Ep2 cells had the same retention time as that shown by promyelocyte inhibitin .
	manualset3
198297	1	416244	7	NULL	NULL	0	NULL	homologous recombination techniques 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using homologous recombination techniques , we successfully generated recombinants of MHV-76 that encode green fluorescent protein ( MHV76-GFP ) and KSHV K1 ( MHV76-K1 ) .
	manualset3
198298	2	416244	7	NULL	NULL	0	NULL	recombinants	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Using homologous recombination techniques , we successfully generated recombinants of MHV-76 that encode green fluorescent protein ( MHV76-GFP ) and KSHV K1 ( MHV76-K1 ) .
	manualset3
198299	3	416244	7	NULL	NULL	0	NULL	MHV-76	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Using homologous recombination techniques , we successfully generated recombinants of MHV-76 that encode green fluorescent protein ( MHV76-GFP ) and KSHV K1 ( MHV76-K1 ) .
	manualset3
198300	4	416244	7	NULL	NULL	0	NULL	green fluorescent protein ( MHV76-GFP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using homologous recombination techniques , we successfully generated recombinants of MHV-76 that encode green fluorescent protein ( MHV76-GFP ) and KSHV K1 ( MHV76-K1 ) .
	manualset3
198301	5	416244	7	NULL	NULL	0	NULL	KSHV K1 ( MHV76-K1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using homologous recombination techniques , we successfully generated recombinants of MHV-76 that encode green fluorescent protein ( MHV76-GFP ) and KSHV K1 ( MHV76-K1 ) .
	manualset3
198302	1	416245	7	NULL	NULL	0	NULL	immunoprecipitation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using immunoprecipitation and co-pelleting assays , we show that the Invs gene product inversin forms a stable complex with tubulin in cultured renal epithelial cells .
	manualset3
198303	2	416245	7	NULL	NULL	0	NULL	co-pelleting assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using immunoprecipitation and co-pelleting assays , we show that the Invs gene product inversin forms a stable complex with tubulin in cultured renal epithelial cells .
	manualset3
198304	3	416245	7	NULL	NULL	0	NULL	Invs gene product	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using immunoprecipitation and co-pelleting assays , we show that the Invs gene product inversin forms a stable complex with tubulin in cultured renal epithelial cells .
	manualset3
198305	4	416245	7	NULL	NULL	0	NULL	inversin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using immunoprecipitation and co-pelleting assays , we show that the Invs gene product inversin forms a stable complex with tubulin in cultured renal epithelial cells .
	manualset3
198306	5	416245	7	NULL	NULL	0	NULL	stable complex 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using immunoprecipitation and co-pelleting assays , we show that the Invs gene product inversin forms a stable complex with tubulin in cultured renal epithelial cells .
	manualset3
198307	6	416245	7	NULL	NULL	0	NULL	tubulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using immunoprecipitation and co-pelleting assays , we show that the Invs gene product inversin forms a stable complex with tubulin in cultured renal epithelial cells .
	manualset3
198308	7	416245	7	NULL	NULL	0	NULL	cultured renal epithelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using immunoprecipitation and co-pelleting assays , we show that the Invs gene product inversin forms a stable complex with tubulin in cultured renal epithelial cells .
	manualset3
198309	1	416246	7	NULL	NULL	0	NULL	inhibitory analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using inhibitory analysis , both PRE1 and PRE2 were shown to belong to serine peptidases .
	manualset3
198310	2	416246	7	NULL	NULL	0	NULL	PRE1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using inhibitory analysis , both PRE1 and PRE2 were shown to belong to serine peptidases .
	manualset3
198311	3	416246	7	NULL	NULL	0	NULL	PRE2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using inhibitory analysis , both PRE1 and PRE2 were shown to belong to serine peptidases .
	manualset3
198312	4	416246	7	NULL	NULL	0	NULL	serine peptidases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using inhibitory analysis , both PRE1 and PRE2 were shown to belong to serine peptidases .
	manualset3
198313	1	416247	7	NULL	NULL	0	NULL	 lectin overlay of protein blots	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using lectin overlay of protein blots and lectin-affinity chromatography , we have found that the major PNA-binding glycoproteins on total as well as on immature ( PNA + ) human thymocytes correspond to two bands of Mr 170 , 000 and 180 , 000 .
	manualset3
198314	2	416247	7	NULL	NULL	0	NULL	 lectin-affinity chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using lectin overlay of protein blots and lectin-affinity chromatography , we have found that the major PNA-binding glycoproteins on total as well as on immature ( PNA + ) human thymocytes correspond to two bands of Mr 170 , 000 and 180 , 000 .
	manualset3
198315	3	416247	7	NULL	NULL	0	NULL	major PNA-binding glycoproteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using lectin overlay of protein blots and lectin-affinity chromatography , we have found that the major PNA-binding glycoproteins on total as well as on immature ( PNA + ) human thymocytes correspond to two bands of Mr 170 , 000 and 180 , 000 .
	manualset3
198316	4	416247	7	NULL	NULL	0	NULL	 total human thymocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using lectin overlay of protein blots and lectin-affinity chromatography , we have found that the major PNA-binding glycoproteins on total as well as on immature ( PNA + ) human thymocytes correspond to two bands of Mr 170 , 000 and 180 , 000 .
	manualset3
198317	5	416247	7	NULL	NULL	0	NULL	immature ( PNA + ) human thymocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using lectin overlay of protein blots and lectin-affinity chromatography , we have found that the major PNA-binding glycoproteins on total as well as on immature ( PNA + ) human thymocytes correspond to two bands of Mr 170 , 000 and 180 , 000 .
	manualset3
198318	6	416247	7	NULL	NULL	0	NULL	two bands	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using lectin overlay of protein blots and lectin-affinity chromatography , we have found that the major PNA-binding glycoproteins on total as well as on immature ( PNA + ) human thymocytes correspond to two bands of Mr 170 , 000 and 180 , 000 .
	manualset3
198319	7	416247	7	NULL	NULL	0	NULL	Mr 170 , 000	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using lectin overlay of protein blots and lectin-affinity chromatography , we have found that the major PNA-binding glycoproteins on total as well as on immature ( PNA + ) human thymocytes correspond to two bands of Mr 170 , 000 and 180 , 000 .
	manualset3
198320	8	416247	7	NULL	NULL	0	NULL	Mr 180 , 000	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using lectin overlay of protein blots and lectin-affinity chromatography , we have found that the major PNA-binding glycoproteins on total as well as on immature ( PNA + ) human thymocytes correspond to two bands of Mr 170 , 000 and 180 , 000 .
	manualset3
198321	1	416248	7	NULL	NULL	0	NULL	 linkage analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using linkage analysis for the F ( 2 ) mapping population consisting of 320 completely male sterile individuals derived from a cross between Pei'ai 64S and 93-11 ( indica restorer ) lines , the pms1 ( t ) gene was delimited to the region between the RM21242 ( 0.2 cM ) and YF11 ( 0.2 cM ) markers on the short arm of chromosome 7 .
	manualset3
198322	2	416248	7	NULL	NULL	NULL	NULL	 F ( 2 ) mapping population	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using linkage analysis for the F ( 2 ) mapping population consisting of 320 completely male sterile individuals derived from a cross between Pei'ai 64S and 93-11 ( indica restorer ) lines , the pms1 ( t ) gene was delimited to the region between the RM21242 ( 0.2 cM ) and YF11 ( 0.2 cM ) markers on the short arm of chromosome 7 .
	manualset3
198323	3	416248	7	NULL	NULL	NULL	NULL	male sterile individuals	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using linkage analysis for the F ( 2 ) mapping population consisting of 320 completely male sterile individuals derived from a cross between Pei'ai 64S and 93-11 ( indica restorer ) lines , the pms1 ( t ) gene was delimited to the region between the RM21242 ( 0.2 cM ) and YF11 ( 0.2 cM ) markers on the short arm of chromosome 7 .
	manualset3
198324	4	416248	7	NULL	NULL	0	NULL	cross	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using linkage analysis for the F ( 2 ) mapping population consisting of 320 completely male sterile individuals derived from a cross between Pei'ai 64S and 93-11 ( indica restorer ) lines , the pms1 ( t ) gene was delimited to the region between the RM21242 ( 0.2 cM ) and YF11 ( 0.2 cM ) markers on the short arm of chromosome 7 .
	manualset3
198325	5	416248	7	NULL	NULL	NULL	NULL	Pei'ai 64S lines	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using linkage analysis for the F ( 2 ) mapping population consisting of 320 completely male sterile individuals derived from a cross between Pei'ai 64S and 93-11 ( indica restorer ) lines , the pms1 ( t ) gene was delimited to the region between the RM21242 ( 0.2 cM ) and YF11 ( 0.2 cM ) markers on the short arm of chromosome 7 .
	manualset3
198326	6	416248	7	NULL	NULL	0	NULL	93-11 ( indica restorer ) lines	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Using linkage analysis for the F ( 2 ) mapping population consisting of 320 completely male sterile individuals derived from a cross between Pei'ai 64S and 93-11 ( indica restorer ) lines , the pms1 ( t ) gene was delimited to the region between the RM21242 ( 0.2 cM ) and YF11 ( 0.2 cM ) markers on the short arm of chromosome 7 .
	manualset3
198327	7	416248	7	NULL	NULL	0	NULL	pms1 ( t ) gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Using linkage analysis for the F ( 2 ) mapping population consisting of 320 completely male sterile individuals derived from a cross between Pei'ai 64S and 93-11 ( indica restorer ) lines , the pms1 ( t ) gene was delimited to the region between the RM21242 ( 0.2 cM ) and YF11 ( 0.2 cM ) markers on the short arm of chromosome 7 .
	manualset3
198328	8	416248	7	NULL	NULL	NULL	NULL	region	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using linkage analysis for the F ( 2 ) mapping population consisting of 320 completely male sterile individuals derived from a cross between Pei'ai 64S and 93-11 ( indica restorer ) lines , the pms1 ( t ) gene was delimited to the region between the RM21242 ( 0.2 cM ) and YF11 ( 0.2 cM ) markers on the short arm of chromosome 7 .
	manualset3
198329	9	416248	7	NULL	NULL	NULL	NULL	RM21242 ( 0.2 cM ) marker	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using linkage analysis for the F ( 2 ) mapping population consisting of 320 completely male sterile individuals derived from a cross between Pei'ai 64S and 93-11 ( indica restorer ) lines , the pms1 ( t ) gene was delimited to the region between the RM21242 ( 0.2 cM ) and YF11 ( 0.2 cM ) markers on the short arm of chromosome 7 .
	manualset3
198330	10	416248	7	NULL	NULL	NULL	NULL	YF11 ( 0.2 cM ) markers	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using linkage analysis for the F ( 2 ) mapping population consisting of 320 completely male sterile individuals derived from a cross between Pei'ai 64S and 93-11 ( indica restorer ) lines , the pms1 ( t ) gene was delimited to the region between the RM21242 ( 0.2 cM ) and YF11 ( 0.2 cM ) markers on the short arm of chromosome 7 .
	manualset3
198331	11	416248	7	NULL	NULL	0	NULL	short arm of chromosome 7 	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Using linkage analysis for the F ( 2 ) mapping population consisting of 320 completely male sterile individuals derived from a cross between Pei'ai 64S and 93-11 ( indica restorer ) lines , the pms1 ( t ) gene was delimited to the region between the RM21242 ( 0.2 cM ) and YF11 ( 0.2 cM ) markers on the short arm of chromosome 7 .
	manualset3
201347	12	416248	7	NULL	NULL	0	NULL	320	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Using linkage analysis for the F ( 2 ) mapping population consisting of 320 completely male sterile individuals derived from a cross between Pei'ai 64S and 93-11 ( indica restorer ) lines , the pms1 ( t ) gene was delimited to the region between the RM21242 ( 0.2 cM ) and YF11 ( 0.2 cM ) markers on the short arm of chromosome 7 .
	manualset3
198332	1	416249	7	NULL	NULL	NULL	NULL	meshes in order	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using meshes in order to strengthen the hiatus of the esophagus is an efficient procedure which reduces the risk of reoccurences .
	manualset3
198333	2	416249	7	NULL	NULL	0	NULL	 hiatus of the esophagus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Using meshes in order to strengthen the hiatus of the esophagus is an efficient procedure which reduces the risk of reoccurences .
	manualset3
198334	3	416249	7	NULL	NULL	0	NULL	efficient procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Using meshes in order to strengthen the hiatus of the esophagus is an efficient procedure which reduces the risk of reoccurences .
	manualset3
198335	4	416249	7	NULL	NULL	0	NULL	 risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using meshes in order to strengthen the hiatus of the esophagus is an efficient procedure which reduces the risk of reoccurences .
	manualset3
198336	5	416249	7	NULL	NULL	0	NULL	 reoccurences	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using meshes in order to strengthen the hiatus of the esophagus is an efficient procedure which reduces the risk of reoccurences .
	manualset3
198337	1	416250	7	NULL	NULL	0	NULL	troglitazone treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After troglitazone treatment GDR improved ( P & lt ; 0.05 ) despite an increase in BMI ( P & lt ; 0.05 ) , whereas metformin had no significant effect on GDR .
	manualset3
198338	2	416250	7	NULL	NULL	0	NULL	GDR	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After troglitazone treatment GDR improved ( P & lt ; 0.05 ) despite an increase in BMI ( P & lt ; 0.05 ) , whereas metformin had no significant effect on GDR .
	manualset3
198339	3	416250	7	NULL	NULL	0	NULL	P & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	After troglitazone treatment GDR improved ( P & lt ; 0.05 ) despite an increase in BMI ( P & lt ; 0.05 ) , whereas metformin had no significant effect on GDR .
	manualset3
198340	4	416250	7	NULL	NULL	0	NULL	BMI	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After troglitazone treatment GDR improved ( P & lt ; 0.05 ) despite an increase in BMI ( P & lt ; 0.05 ) , whereas metformin had no significant effect on GDR .
	manualset3
198341	5	416250	7	NULL	NULL	0	NULL	P & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	After troglitazone treatment GDR improved ( P & lt ; 0.05 ) despite an increase in BMI ( P & lt ; 0.05 ) , whereas metformin had no significant effect on GDR .
	manualset3
198342	6	416250	7	NULL	NULL	0	NULL	metformin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	After troglitazone treatment GDR improved ( P & lt ; 0.05 ) despite an increase in BMI ( P & lt ; 0.05 ) , whereas metformin had no significant effect on GDR .
	manualset3
198343	7	416250	7	NULL	NULL	0	NULL	no significant effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After troglitazone treatment GDR improved ( P & lt ; 0.05 ) despite an increase in BMI ( P & lt ; 0.05 ) , whereas metformin had no significant effect on GDR .
	manualset3
198344	8	416250	7	NULL	NULL	0	NULL	GDR	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After troglitazone treatment GDR improved ( P & lt ; 0.05 ) despite an increase in BMI ( P & lt ; 0.05 ) , whereas metformin had no significant effect on GDR .
	manualset3
198610	1	416251	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Using mice deficient in interleukin-6 ( IL-6 ) , the role of IL-6 in the regulation of hepatic CYP activity , glutathione ( GSH ) metabolism , and catalase ( CAT ) activity was analyzed after LPS administration .
	manualset3
198611	2	416251	7	NULL	NULL	0	NULL	interleukin-6 ( IL-6 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using mice deficient in interleukin-6 ( IL-6 ) , the role of IL-6 in the regulation of hepatic CYP activity , glutathione ( GSH ) metabolism , and catalase ( CAT ) activity was analyzed after LPS administration .
	manualset3
198612	3	416251	7	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using mice deficient in interleukin-6 ( IL-6 ) , the role of IL-6 in the regulation of hepatic CYP activity , glutathione ( GSH ) metabolism , and catalase ( CAT ) activity was analyzed after LPS administration .
	manualset3
198613	4	416251	7	NULL	NULL	0	NULL	 IL-6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using mice deficient in interleukin-6 ( IL-6 ) , the role of IL-6 in the regulation of hepatic CYP activity , glutathione ( GSH ) metabolism , and catalase ( CAT ) activity was analyzed after LPS administration .
	manualset3
198614	5	416251	7	NULL	NULL	0	NULL	regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using mice deficient in interleukin-6 ( IL-6 ) , the role of IL-6 in the regulation of hepatic CYP activity , glutathione ( GSH ) metabolism , and catalase ( CAT ) activity was analyzed after LPS administration .
	manualset3
198615	6	416251	7	NULL	NULL	NULL	NULL	hepatic CYP activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using mice deficient in interleukin-6 ( IL-6 ) , the role of IL-6 in the regulation of hepatic CYP activity , glutathione ( GSH ) metabolism , and catalase ( CAT ) activity was analyzed after LPS administration .
	manualset3
198616	7	416251	7	NULL	NULL	0	NULL	 glutathione ( GSH ) metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using mice deficient in interleukin-6 ( IL-6 ) , the role of IL-6 in the regulation of hepatic CYP activity , glutathione ( GSH ) metabolism , and catalase ( CAT ) activity was analyzed after LPS administration .
	manualset3
198617	8	416251	7	NULL	NULL	0	NULL	catalase ( CAT ) activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using mice deficient in interleukin-6 ( IL-6 ) , the role of IL-6 in the regulation of hepatic CYP activity , glutathione ( GSH ) metabolism , and catalase ( CAT ) activity was analyzed after LPS administration .
	manualset3
198618	9	416251	7	NULL	NULL	0	NULL	LPS administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Using mice deficient in interleukin-6 ( IL-6 ) , the role of IL-6 in the regulation of hepatic CYP activity , glutathione ( GSH ) metabolism , and catalase ( CAT ) activity was analyzed after LPS administration .
	manualset3
198619	1	416252	7	NULL	NULL	0	NULL	molecular dynamics simulations	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Using molecular dynamics simulations we study , in two dimensions , the temperature-density phase diagram of a simple model with two internal states labeled 1 and -1 .
	manualset3
198620	2	416252	7	NULL	NULL	0	NULL	two dimensions	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using molecular dynamics simulations we study , in two dimensions , the temperature-density phase diagram of a simple model with two internal states labeled 1 and -1 .
	manualset3
198621	3	416252	7	NULL	NULL	0	NULL	temperature-density phase diagram 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Using molecular dynamics simulations we study , in two dimensions , the temperature-density phase diagram of a simple model with two internal states labeled 1 and -1 .
	manualset3
198622	4	416252	7	NULL	NULL	0	NULL	 simple model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Using molecular dynamics simulations we study , in two dimensions , the temperature-density phase diagram of a simple model with two internal states labeled 1 and -1 .
	manualset3
198623	5	416252	7	NULL	NULL	0	NULL	two internal states	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using molecular dynamics simulations we study , in two dimensions , the temperature-density phase diagram of a simple model with two internal states labeled 1 and -1 .
	manualset3
198624	6	416252	7	NULL	NULL	0	NULL	1	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using molecular dynamics simulations we study , in two dimensions , the temperature-density phase diagram of a simple model with two internal states labeled 1 and -1 .
	manualset3
198625	7	416252	7	NULL	NULL	0	NULL	 -1	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using molecular dynamics simulations we study , in two dimensions , the temperature-density phase diagram of a simple model with two internal states labeled 1 and -1 .
	manualset3
198626	1	416253	7	NULL	NULL	0	NULL	nationally representative data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Using nationally representative data on young people ( 15-24 ) from Burkina Faso , Ghana and Zambia , the analysis examines the economic , demographic and behavioral dimensions of community environments that shape HIV-related stigma among young people .
	manualset3
198627	2	416253	7	NULL	NULL	0	NULL	young people ( 15-24 )	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using nationally representative data on young people ( 15-24 ) from Burkina Faso , Ghana and Zambia , the analysis examines the economic , demographic and behavioral dimensions of community environments that shape HIV-related stigma among young people .
	manualset3
198628	3	416253	7	NULL	NULL	0	NULL	Burkina Faso	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Using nationally representative data on young people ( 15-24 ) from Burkina Faso , Ghana and Zambia , the analysis examines the economic , demographic and behavioral dimensions of community environments that shape HIV-related stigma among young people .
	manualset3
198629	4	416253	7	NULL	NULL	0	NULL	Ghana	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Using nationally representative data on young people ( 15-24 ) from Burkina Faso , Ghana and Zambia , the analysis examines the economic , demographic and behavioral dimensions of community environments that shape HIV-related stigma among young people .
	manualset3
198630	5	416253	7	NULL	NULL	0	NULL	 Zambia	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Using nationally representative data on young people ( 15-24 ) from Burkina Faso , Ghana and Zambia , the analysis examines the economic , demographic and behavioral dimensions of community environments that shape HIV-related stigma among young people .
	manualset3
198631	6	416253	7	NULL	NULL	0	NULL	 analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using nationally representative data on young people ( 15-24 ) from Burkina Faso , Ghana and Zambia , the analysis examines the economic , demographic and behavioral dimensions of community environments that shape HIV-related stigma among young people .
	manualset3
198632	7	416253	7	NULL	NULL	0	NULL	economic dimension	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using nationally representative data on young people ( 15-24 ) from Burkina Faso , Ghana and Zambia , the analysis examines the economic , demographic and behavioral dimensions of community environments that shape HIV-related stigma among young people .
	manualset3
198633	8	416253	7	NULL	NULL	0	NULL	demographic dimension	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using nationally representative data on young people ( 15-24 ) from Burkina Faso , Ghana and Zambia , the analysis examines the economic , demographic and behavioral dimensions of community environments that shape HIV-related stigma among young people .
	manualset3
198634	9	416253	7	NULL	NULL	0	NULL	behavioral dimensions	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using nationally representative data on young people ( 15-24 ) from Burkina Faso , Ghana and Zambia , the analysis examines the economic , demographic and behavioral dimensions of community environments that shape HIV-related stigma among young people .
	manualset3
198635	10	416253	7	NULL	NULL	0	NULL	community environments	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Using nationally representative data on young people ( 15-24 ) from Burkina Faso , Ghana and Zambia , the analysis examines the economic , demographic and behavioral dimensions of community environments that shape HIV-related stigma among young people .
	manualset3
198636	11	416253	7	NULL	NULL	0	NULL	HIV-related stigma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using nationally representative data on young people ( 15-24 ) from Burkina Faso , Ghana and Zambia , the analysis examines the economic , demographic and behavioral dimensions of community environments that shape HIV-related stigma among young people .
	manualset3
198637	12	416253	7	NULL	NULL	0	NULL	young people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using nationally representative data on young people ( 15-24 ) from Burkina Faso , Ghana and Zambia , the analysis examines the economic , demographic and behavioral dimensions of community environments that shape HIV-related stigma among young people .
	manualset3
198638	1	416254	7	NULL	NULL	0	NULL	open ghost membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Using open ghost membranes prepared from sickle RBC , we examined the ability of membrane-associated Fe ( III ) to resist removal by 15 chelators representing a 40-log range of affinities for Fe ( III ) .
	manualset3
198639	2	416254	7	NULL	NULL	0	NULL	sickle RBC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using open ghost membranes prepared from sickle RBC , we examined the ability of membrane-associated Fe ( III ) to resist removal by 15 chelators representing a 40-log range of affinities for Fe ( III ) .
	manualset3
198640	3	416254	7	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using open ghost membranes prepared from sickle RBC , we examined the ability of membrane-associated Fe ( III ) to resist removal by 15 chelators representing a 40-log range of affinities for Fe ( III ) .
	manualset3
198641	4	416254	7	NULL	NULL	0	NULL	membrane-associated Fe ( III )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using open ghost membranes prepared from sickle RBC , we examined the ability of membrane-associated Fe ( III ) to resist removal by 15 chelators representing a 40-log range of affinities for Fe ( III ) .
	manualset3
198642	5	416254	7	NULL	NULL	0	NULL	removal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using open ghost membranes prepared from sickle RBC , we examined the ability of membrane-associated Fe ( III ) to resist removal by 15 chelators representing a 40-log range of affinities for Fe ( III ) .
	manualset3
198643	6	416254	7	NULL	NULL	0	NULL	15 chelators	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using open ghost membranes prepared from sickle RBC , we examined the ability of membrane-associated Fe ( III ) to resist removal by 15 chelators representing a 40-log range of affinities for Fe ( III ) .
	manualset3
198644	7	416254	7	NULL	NULL	0	NULL	40-log range 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using open ghost membranes prepared from sickle RBC , we examined the ability of membrane-associated Fe ( III ) to resist removal by 15 chelators representing a 40-log range of affinities for Fe ( III ) .
	manualset3
198645	9	416254	7	NULL	NULL	NULL	NULL	Fe ( III )	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using open ghost membranes prepared from sickle RBC , we examined the ability of membrane-associated Fe ( III ) to resist removal by 15 chelators representing a 40-log range of affinities for Fe ( III ) .
	manualset3
198646	8	416254	7	NULL	NULL	0	NULL	affinities 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using open ghost membranes prepared from sickle RBC , we examined the ability of membrane-associated Fe ( III ) to resist removal by 15 chelators representing a 40-log range of affinities for Fe ( III ) .
	manualset3
198647	1	416255	7	NULL	NULL	0	NULL	optimized DTI methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using optimized DTI methods on a cohort of 121 right-handed children and adults aged 6-68 years , we examined the CC areas and corresponding DTI metrics of the different functionally specialized sectors of the CC .
	manualset3
198648	2	416255	7	NULL	NULL	0	NULL	cohort 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using optimized DTI methods on a cohort of 121 right-handed children and adults aged 6-68 years , we examined the CC areas and corresponding DTI metrics of the different functionally specialized sectors of the CC .
	manualset3
198649	3	416255	7	NULL	NULL	0	NULL	121 right-handed children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using optimized DTI methods on a cohort of 121 right-handed children and adults aged 6-68 years , we examined the CC areas and corresponding DTI metrics of the different functionally specialized sectors of the CC .
	manualset3
198650	4	416255	7	NULL	NULL	NULL	NULL	 adults	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using optimized DTI methods on a cohort of 121 right-handed children and adults aged 6-68 years , we examined the CC areas and corresponding DTI metrics of the different functionally specialized sectors of the CC .
	manualset3
198651	5	416255	7	NULL	NULL	0	NULL	aged 6-68 years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Using optimized DTI methods on a cohort of 121 right-handed children and adults aged 6-68 years , we examined the CC areas and corresponding DTI metrics of the different functionally specialized sectors of the CC .
	manualset3
198652	6	416255	7	NULL	NULL	0	NULL	CC areas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Using optimized DTI methods on a cohort of 121 right-handed children and adults aged 6-68 years , we examined the CC areas and corresponding DTI metrics of the different functionally specialized sectors of the CC .
	manualset3
198653	7	416255	7	NULL	NULL	0	NULL	DTI metrics 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using optimized DTI methods on a cohort of 121 right-handed children and adults aged 6-68 years , we examined the CC areas and corresponding DTI metrics of the different functionally specialized sectors of the CC .
	manualset3
198654	8	416255	7	NULL	NULL	0	NULL	functionally specialized sectors	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Using optimized DTI methods on a cohort of 121 right-handed children and adults aged 6-68 years , we examined the CC areas and corresponding DTI metrics of the different functionally specialized sectors of the CC .
	manualset3
198655	9	416255	7	NULL	NULL	0	NULL	CC	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Using optimized DTI methods on a cohort of 121 right-handed children and adults aged 6-68 years , we examined the CC areas and corresponding DTI metrics of the different functionally specialized sectors of the CC .
	manualset3
198656	1	416256	7	NULL	NULL	0	NULL	pCMVbeta	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Using pCMVbeta as a model gene , the biodistribution of plasmid DNA was measured by quantitative polymerase chain reaction .
	manualset3
198657	2	416256	7	NULL	NULL	0	NULL	 model gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Using pCMVbeta as a model gene , the biodistribution of plasmid DNA was measured by quantitative polymerase chain reaction .
	manualset3
198658	3	416256	7	NULL	NULL	0	NULL	biodistribution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using pCMVbeta as a model gene , the biodistribution of plasmid DNA was measured by quantitative polymerase chain reaction .
	manualset3
198659	4	416256	7	NULL	NULL	0	NULL	plasmid DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using pCMVbeta as a model gene , the biodistribution of plasmid DNA was measured by quantitative polymerase chain reaction .
	manualset3
198660	5	416256	7	NULL	NULL	0	NULL	 quantitative polymerase chain reaction 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using pCMVbeta as a model gene , the biodistribution of plasmid DNA was measured by quantitative polymerase chain reaction .
	manualset3
198661	1	416257	7	NULL	NULL	0	NULL	polymerase chain reaction-restriction fragment length polymorphism ( PCR-RFLP )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using polymerase chain reaction-restriction fragment length polymorphism ( PCR-RFLP ) , two genotypes were found at each site , which were ins/del and ins/ins at locus -753 , and A/A and A/G at locus -391 , respectively .
	manualset3
198662	2	416257	7	NULL	NULL	0	NULL	 two genotypes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using polymerase chain reaction-restriction fragment length polymorphism ( PCR-RFLP ) , two genotypes were found at each site , which were ins/del and ins/ins at locus -753 , and A/A and A/G at locus -391 , respectively .
	manualset3
198663	3	416257	7	NULL	NULL	0	NULL	site	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using polymerase chain reaction-restriction fragment length polymorphism ( PCR-RFLP ) , two genotypes were found at each site , which were ins/del and ins/ins at locus -753 , and A/A and A/G at locus -391 , respectively .
	manualset3
198664	4	416257	7	NULL	NULL	0	NULL	ins/del	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using polymerase chain reaction-restriction fragment length polymorphism ( PCR-RFLP ) , two genotypes were found at each site , which were ins/del and ins/ins at locus -753 , and A/A and A/G at locus -391 , respectively .
	manualset3
198665	5	416257	7	NULL	NULL	0	NULL	ins/ins	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using polymerase chain reaction-restriction fragment length polymorphism ( PCR-RFLP ) , two genotypes were found at each site , which were ins/del and ins/ins at locus -753 , and A/A and A/G at locus -391 , respectively .
	manualset3
198666	6	416257	7	NULL	NULL	0	NULL	locus -753	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Using polymerase chain reaction-restriction fragment length polymorphism ( PCR-RFLP ) , two genotypes were found at each site , which were ins/del and ins/ins at locus -753 , and A/A and A/G at locus -391 , respectively .
	manualset3
198667	7	416257	7	NULL	NULL	0	NULL	A/A locus	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Using polymerase chain reaction-restriction fragment length polymorphism ( PCR-RFLP ) , two genotypes were found at each site , which were ins/del and ins/ins at locus -753 , and A/A and A/G at locus -391 , respectively .
	manualset3
198668	8	416257	7	NULL	NULL	0	NULL	A/G locus	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Using polymerase chain reaction-restriction fragment length polymorphism ( PCR-RFLP ) , two genotypes were found at each site , which were ins/del and ins/ins at locus -753 , and A/A and A/G at locus -391 , respectively .
	manualset3
198669	9	416257	7	NULL	NULL	0	NULL	locus -391	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Using polymerase chain reaction-restriction fragment length polymorphism ( PCR-RFLP ) , two genotypes were found at each site , which were ins/del and ins/ins at locus -753 , and A/A and A/G at locus -391 , respectively .
	manualset3
198670	1	416258	7	NULL	NULL	0	NULL	principles 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using principles of evidence-based medicine , we observed that none of the medical treatments proved efficiency on preventing vascular thrombosis , arterial or venous .
	manualset3
198671	2	416258	7	NULL	NULL	0	NULL	evidence-based medicine	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Using principles of evidence-based medicine , we observed that none of the medical treatments proved efficiency on preventing vascular thrombosis , arterial or venous .
	manualset3
198672	3	416258	7	NULL	NULL	0	NULL	medical treatments	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Using principles of evidence-based medicine , we observed that none of the medical treatments proved efficiency on preventing vascular thrombosis , arterial or venous .
	manualset3
198673	4	416258	7	NULL	NULL	0	NULL	preventing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using principles of evidence-based medicine , we observed that none of the medical treatments proved efficiency on preventing vascular thrombosis , arterial or venous .
	manualset3
198674	5	416258	7	NULL	NULL	0	NULL	vascular thrombosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using principles of evidence-based medicine , we observed that none of the medical treatments proved efficiency on preventing vascular thrombosis , arterial or venous .
	manualset3
198675	6	416258	7	NULL	NULL	0	NULL	arterial thrombosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using principles of evidence-based medicine , we observed that none of the medical treatments proved efficiency on preventing vascular thrombosis , arterial or venous .
	manualset3
198676	7	416258	7	NULL	NULL	0	NULL	venous thrombosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using principles of evidence-based medicine , we observed that none of the medical treatments proved efficiency on preventing vascular thrombosis , arterial or venous .
	manualset3
198677	1	416259	7	NULL	NULL	0	NULL	truncation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After truncation and filtering of the VUSE pulse in the time domain , the general shape of the VUSE RF excitation profile is maintained , but the maximum flip angle is reduced .
	manualset3
198678	2	416259	7	NULL	NULL	0	NULL	filtering	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After truncation and filtering of the VUSE pulse in the time domain , the general shape of the VUSE RF excitation profile is maintained , but the maximum flip angle is reduced .
	manualset3
198679	3	416259	7	NULL	NULL	0	NULL	VUSE pulse	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	After truncation and filtering of the VUSE pulse in the time domain , the general shape of the VUSE RF excitation profile is maintained , but the maximum flip angle is reduced .
	manualset3
198680	4	416259	7	NULL	NULL	0	NULL	time domain	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	After truncation and filtering of the VUSE pulse in the time domain , the general shape of the VUSE RF excitation profile is maintained , but the maximum flip angle is reduced .
	manualset3
198681	5	416259	7	NULL	NULL	0	NULL	general shape	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	After truncation and filtering of the VUSE pulse in the time domain , the general shape of the VUSE RF excitation profile is maintained , but the maximum flip angle is reduced .
	manualset3
198682	6	416259	7	NULL	NULL	0	NULL	VUSE RF excitation profile	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	After truncation and filtering of the VUSE pulse in the time domain , the general shape of the VUSE RF excitation profile is maintained , but the maximum flip angle is reduced .
	manualset3
198683	7	416259	7	NULL	NULL	0	NULL	maximum flip angle	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After truncation and filtering of the VUSE pulse in the time domain , the general shape of the VUSE RF excitation profile is maintained , but the maximum flip angle is reduced .
	manualset3
198684	1	416260	7	NULL	NULL	0	NULL	rabies virus infection	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Using rabies virus infection as an example , we discuss the advances in passive immunoprophylaxis , most notably the shift from the recommended polyclonal human or equine immunoglobulins to monoclonal antibody therapies .
	manualset3
198685	2	416260	7	NULL	NULL	0	NULL	example	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Using rabies virus infection as an example , we discuss the advances in passive immunoprophylaxis , most notably the shift from the recommended polyclonal human or equine immunoglobulins to monoclonal antibody therapies .
	manualset3
198686	3	416260	7	NULL	NULL	0	NULL	advances	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using rabies virus infection as an example , we discuss the advances in passive immunoprophylaxis , most notably the shift from the recommended polyclonal human or equine immunoglobulins to monoclonal antibody therapies .
	manualset3
198687	4	416260	7	NULL	NULL	0	NULL	passive immunoprophylaxis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using rabies virus infection as an example , we discuss the advances in passive immunoprophylaxis , most notably the shift from the recommended polyclonal human or equine immunoglobulins to monoclonal antibody therapies .
	manualset3
198688	5	416260	7	NULL	NULL	0	NULL	shift	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using rabies virus infection as an example , we discuss the advances in passive immunoprophylaxis , most notably the shift from the recommended polyclonal human or equine immunoglobulins to monoclonal antibody therapies .
	manualset3
198689	6	416260	7	NULL	NULL	0	NULL	recommended polyclonal human immunoglobulins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using rabies virus infection as an example , we discuss the advances in passive immunoprophylaxis , most notably the shift from the recommended polyclonal human or equine immunoglobulins to monoclonal antibody therapies .
	manualset3
198690	7	416260	7	NULL	NULL	0	NULL	equine immunoglobulins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using rabies virus infection as an example , we discuss the advances in passive immunoprophylaxis , most notably the shift from the recommended polyclonal human or equine immunoglobulins to monoclonal antibody therapies .
	manualset3
198691	8	416260	7	NULL	NULL	0	NULL	monoclonal antibody therapies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Using rabies virus infection as an example , we discuss the advances in passive immunoprophylaxis , most notably the shift from the recommended polyclonal human or equine immunoglobulins to monoclonal antibody therapies .
	manualset3
198692	1	416261	7	NULL	NULL	0	NULL	radioactive tracers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using radioactive tracers , the effect of n-alkanes with a varying length -- C16-C25 -- of the carbon chain on the rate of yeast growth and the ratio of major chemicals in their biomass was studied .
	manualset3
198693	2	416261	7	NULL	NULL	0	NULL	effect 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using radioactive tracers , the effect of n-alkanes with a varying length -- C16-C25 -- of the carbon chain on the rate of yeast growth and the ratio of major chemicals in their biomass was studied .
	manualset3
198694	3	416261	7	NULL	NULL	0	NULL	 n-alkanes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using radioactive tracers , the effect of n-alkanes with a varying length -- C16-C25 -- of the carbon chain on the rate of yeast growth and the ratio of major chemicals in their biomass was studied .
	manualset3
198695	4	416261	7	NULL	NULL	0	NULL	varying length	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using radioactive tracers , the effect of n-alkanes with a varying length -- C16-C25 -- of the carbon chain on the rate of yeast growth and the ratio of major chemicals in their biomass was studied .
	manualset3
198696	5	416261	7	NULL	NULL	0	NULL	 C16-C25 --	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using radioactive tracers , the effect of n-alkanes with a varying length -- C16-C25 -- of the carbon chain on the rate of yeast growth and the ratio of major chemicals in their biomass was studied .
	manualset3
198697	6	416261	7	NULL	NULL	0	NULL	 carbon chain	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using radioactive tracers , the effect of n-alkanes with a varying length -- C16-C25 -- of the carbon chain on the rate of yeast growth and the ratio of major chemicals in their biomass was studied .
	manualset3
198698	7	416261	7	NULL	NULL	0	NULL	rate 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using radioactive tracers , the effect of n-alkanes with a varying length -- C16-C25 -- of the carbon chain on the rate of yeast growth and the ratio of major chemicals in their biomass was studied .
	manualset3
198699	8	416261	7	NULL	NULL	0	NULL	yeast growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using radioactive tracers , the effect of n-alkanes with a varying length -- C16-C25 -- of the carbon chain on the rate of yeast growth and the ratio of major chemicals in their biomass was studied .
	manualset3
198700	9	416261	7	NULL	NULL	0	NULL	 ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using radioactive tracers , the effect of n-alkanes with a varying length -- C16-C25 -- of the carbon chain on the rate of yeast growth and the ratio of major chemicals in their biomass was studied .
	manualset3
198701	10	416261	7	NULL	NULL	0	NULL	major chemicals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using radioactive tracers , the effect of n-alkanes with a varying length -- C16-C25 -- of the carbon chain on the rate of yeast growth and the ratio of major chemicals in their biomass was studied .
	manualset3
198702	11	416261	7	NULL	NULL	NULL	NULL	biomass	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using radioactive tracers , the effect of n-alkanes with a varying length -- C16-C25 -- of the carbon chain on the rate of yeast growth and the ratio of major chemicals in their biomass was studied .
	manualset3
198703	1	416262	7	NULL	NULL	NULL	NULL	 reverse genetics	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using reverse genetics , recombinant RSV ( rRSV ) strains were engineered with truncations at amino acid 118 , 174 , 193 , or 213 and respectively designated rA2cpDeltaG118 , rA2cpDeltaG174 , rA2cpDeltaG193 , and rA2cpDeltaG213 .
	manualset3
198704	2	416262	7	NULL	NULL	0	NULL	recombinant RSV ( rRSV ) strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Using reverse genetics , recombinant RSV ( rRSV ) strains were engineered with truncations at amino acid 118 , 174 , 193 , or 213 and respectively designated rA2cpDeltaG118 , rA2cpDeltaG174 , rA2cpDeltaG193 , and rA2cpDeltaG213 .
	manualset3
198705	3	416262	7	NULL	NULL	NULL	NULL	 truncations	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using reverse genetics , recombinant RSV ( rRSV ) strains were engineered with truncations at amino acid 118 , 174 , 193 , or 213 and respectively designated rA2cpDeltaG118 , rA2cpDeltaG174 , rA2cpDeltaG193 , and rA2cpDeltaG213 .
	manualset3
198706	4	416262	7	NULL	NULL	0	NULL	amino acid 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using reverse genetics , recombinant RSV ( rRSV ) strains were engineered with truncations at amino acid 118 , 174 , 193 , or 213 and respectively designated rA2cpDeltaG118 , rA2cpDeltaG174 , rA2cpDeltaG193 , and rA2cpDeltaG213 .
	manualset3
198707	5	416262	7	NULL	NULL	0	NULL	118	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Using reverse genetics , recombinant RSV ( rRSV ) strains were engineered with truncations at amino acid 118 , 174 , 193 , or 213 and respectively designated rA2cpDeltaG118 , rA2cpDeltaG174 , rA2cpDeltaG193 , and rA2cpDeltaG213 .
	manualset3
198708	6	416262	7	NULL	NULL	0	NULL	174	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Using reverse genetics , recombinant RSV ( rRSV ) strains were engineered with truncations at amino acid 118 , 174 , 193 , or 213 and respectively designated rA2cpDeltaG118 , rA2cpDeltaG174 , rA2cpDeltaG193 , and rA2cpDeltaG213 .
	manualset3
198709	7	416262	7	NULL	NULL	0	NULL	193	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Using reverse genetics , recombinant RSV ( rRSV ) strains were engineered with truncations at amino acid 118 , 174 , 193 , or 213 and respectively designated rA2cpDeltaG118 , rA2cpDeltaG174 , rA2cpDeltaG193 , and rA2cpDeltaG213 .
	manualset3
198710	8	416262	7	NULL	NULL	0	NULL	213	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Using reverse genetics , recombinant RSV ( rRSV ) strains were engineered with truncations at amino acid 118 , 174 , 193 , or 213 and respectively designated rA2cpDeltaG118 , rA2cpDeltaG174 , rA2cpDeltaG193 , and rA2cpDeltaG213 .
	manualset3
198711	9	416262	7	NULL	NULL	0	NULL	rA2cpDeltaG118	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using reverse genetics , recombinant RSV ( rRSV ) strains were engineered with truncations at amino acid 118 , 174 , 193 , or 213 and respectively designated rA2cpDeltaG118 , rA2cpDeltaG174 , rA2cpDeltaG193 , and rA2cpDeltaG213 .
	manualset3
198712	10	416262	7	NULL	NULL	0	NULL	rA2cpDeltaG174	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using reverse genetics , recombinant RSV ( rRSV ) strains were engineered with truncations at amino acid 118 , 174 , 193 , or 213 and respectively designated rA2cpDeltaG118 , rA2cpDeltaG174 , rA2cpDeltaG193 , and rA2cpDeltaG213 .
	manualset3
198713	11	416262	7	NULL	NULL	0	NULL	rA2cpDeltaG193	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using reverse genetics , recombinant RSV ( rRSV ) strains were engineered with truncations at amino acid 118 , 174 , 193 , or 213 and respectively designated rA2cpDeltaG118 , rA2cpDeltaG174 , rA2cpDeltaG193 , and rA2cpDeltaG213 .
	manualset3
198714	12	416262	7	NULL	NULL	0	NULL	rA2cpDeltaG213	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using reverse genetics , recombinant RSV ( rRSV ) strains were engineered with truncations at amino acid 118 , 174 , 193 , or 213 and respectively designated rA2cpDeltaG118 , rA2cpDeltaG174 , rA2cpDeltaG193 , and rA2cpDeltaG213 .
	manualset3
198715	1	416263	7	NULL	NULL	NULL	NULL	reverse genetics	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using reverse genetics , the analogous phenylalanine at position 456 in the L protein of wild-type PIV3 was mutagenized to leucine ( F456L ) .
	manualset3
198716	2	416263	7	NULL	NULL	0	NULL	analogous phenylalanine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using reverse genetics , the analogous phenylalanine at position 456 in the L protein of wild-type PIV3 was mutagenized to leucine ( F456L ) .
	manualset3
198717	3	416263	7	NULL	NULL	0	NULL	 position 456	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using reverse genetics , the analogous phenylalanine at position 456 in the L protein of wild-type PIV3 was mutagenized to leucine ( F456L ) .
	manualset3
198718	4	416263	7	NULL	NULL	0	NULL	L protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using reverse genetics , the analogous phenylalanine at position 456 in the L protein of wild-type PIV3 was mutagenized to leucine ( F456L ) .
	manualset3
198719	5	416263	7	NULL	NULL	0	NULL	wild-type PIV3	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using reverse genetics , the analogous phenylalanine at position 456 in the L protein of wild-type PIV3 was mutagenized to leucine ( F456L ) .
	manualset3
198720	6	416263	7	NULL	NULL	0	NULL	leucine ( F456L )	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using reverse genetics , the analogous phenylalanine at position 456 in the L protein of wild-type PIV3 was mutagenized to leucine ( F456L ) .
	manualset3
198721	1	416264	7	NULL	NULL	0	NULL	self-reported prenatal exposure	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Using self-reported prenatal exposure resulted in non-differential exposure misclassification of SHS exposures that attenuated the association between SHS exposure and BMI compared with serum cotinine concentrations .
	manualset3
198722	2	416264	7	NULL	NULL	0	NULL	non-differential exposure	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Using self-reported prenatal exposure resulted in non-differential exposure misclassification of SHS exposures that attenuated the association between SHS exposure and BMI compared with serum cotinine concentrations .
	manualset3
198723	3	416264	7	NULL	NULL	0	NULL	 misclassification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using self-reported prenatal exposure resulted in non-differential exposure misclassification of SHS exposures that attenuated the association between SHS exposure and BMI compared with serum cotinine concentrations .
	manualset3
198724	4	416264	7	NULL	NULL	0	NULL	SHS exposures	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Using self-reported prenatal exposure resulted in non-differential exposure misclassification of SHS exposures that attenuated the association between SHS exposure and BMI compared with serum cotinine concentrations .
	manualset3
198725	5	416264	7	NULL	NULL	0	NULL	 association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Using self-reported prenatal exposure resulted in non-differential exposure misclassification of SHS exposures that attenuated the association between SHS exposure and BMI compared with serum cotinine concentrations .
	manualset3
198726	6	416264	7	NULL	NULL	0	NULL	SHS exposure	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Using self-reported prenatal exposure resulted in non-differential exposure misclassification of SHS exposures that attenuated the association between SHS exposure and BMI compared with serum cotinine concentrations .
	manualset3
198727	7	416264	7	NULL	NULL	0	NULL	BMI 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using self-reported prenatal exposure resulted in non-differential exposure misclassification of SHS exposures that attenuated the association between SHS exposure and BMI compared with serum cotinine concentrations .
	manualset3
198728	8	416264	7	NULL	NULL	0	NULL	serum cotinine concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using self-reported prenatal exposure resulted in non-differential exposure misclassification of SHS exposures that attenuated the association between SHS exposure and BMI compared with serum cotinine concentrations .
	manualset3
198729	1	416265	7	NULL	NULL	0	NULL	14C-labelled derivatives	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using some 14C-labelled derivatives of cinnamic acid which are of interest as metabolites of chlorogenic acid we studied their pharmacokinetic behavior in rats .
	manualset3
198730	2	416265	7	NULL	NULL	0	NULL	cinnamic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using some 14C-labelled derivatives of cinnamic acid which are of interest as metabolites of chlorogenic acid we studied their pharmacokinetic behavior in rats .
	manualset3
198731	3	416265	7	NULL	NULL	0	NULL	metabolites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using some 14C-labelled derivatives of cinnamic acid which are of interest as metabolites of chlorogenic acid we studied their pharmacokinetic behavior in rats .
	manualset3
198732	4	416265	7	NULL	NULL	0	NULL	chlorogenic acid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using some 14C-labelled derivatives of cinnamic acid which are of interest as metabolites of chlorogenic acid we studied their pharmacokinetic behavior in rats .
	manualset3
198733	5	416265	7	NULL	NULL	0	NULL	pharmacokinetic behavior 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using some 14C-labelled derivatives of cinnamic acid which are of interest as metabolites of chlorogenic acid we studied their pharmacokinetic behavior in rats .
	manualset3
198734	6	416265	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Using some 14C-labelled derivatives of cinnamic acid which are of interest as metabolites of chlorogenic acid we studied their pharmacokinetic behavior in rats .
	manualset3
198735	1	416266	7	NULL	NULL	0	NULL	spin probes-stearic acid analogs 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using spin probes-stearic acid analogs , the authors investigated the microviscosity and the a/b parameter of red blood cell membranes in children with diabetes mellitus .
	manualset3
198736	2	416266	7	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using spin probes-stearic acid analogs , the authors investigated the microviscosity and the a/b parameter of red blood cell membranes in children with diabetes mellitus .
	manualset3
198737	3	416266	7	NULL	NULL	0	NULL	microviscosity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using spin probes-stearic acid analogs , the authors investigated the microviscosity and the a/b parameter of red blood cell membranes in children with diabetes mellitus .
	manualset3
198738	4	416266	7	NULL	NULL	0	NULL	a/b parameter	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Using spin probes-stearic acid analogs , the authors investigated the microviscosity and the a/b parameter of red blood cell membranes in children with diabetes mellitus .
	manualset3
198739	5	416266	7	NULL	NULL	0	NULL	 red blood cell membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Using spin probes-stearic acid analogs , the authors investigated the microviscosity and the a/b parameter of red blood cell membranes in children with diabetes mellitus .
	manualset3
198740	6	416266	7	NULL	NULL	0	NULL	 children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using spin probes-stearic acid analogs , the authors investigated the microviscosity and the a/b parameter of red blood cell membranes in children with diabetes mellitus .
	manualset3
198741	7	416266	7	NULL	NULL	0	NULL	diabetes mellitus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Using spin probes-stearic acid analogs , the authors investigated the microviscosity and the a/b parameter of red blood cell membranes in children with diabetes mellitus .
	manualset3
198742	1	416267	7	NULL	NULL	0	NULL	 statistical analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using statistical analyses for association of MCP3 polymorphisms with asthma development and asthma-related phenotypes , no significant signals were detected .
	manualset3
198743	2	416267	7	NULL	NULL	0	NULL	 association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Using statistical analyses for association of MCP3 polymorphisms with asthma development and asthma-related phenotypes , no significant signals were detected .
	manualset3
198744	3	416267	7	NULL	NULL	0	NULL	MCP3 polymorphisms 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using statistical analyses for association of MCP3 polymorphisms with asthma development and asthma-related phenotypes , no significant signals were detected .
	manualset3
198745	4	416267	7	NULL	NULL	0	NULL	asthma development	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using statistical analyses for association of MCP3 polymorphisms with asthma development and asthma-related phenotypes , no significant signals were detected .
	manualset3
198746	5	416267	7	NULL	NULL	0	NULL	asthma-related phenotypes	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using statistical analyses for association of MCP3 polymorphisms with asthma development and asthma-related phenotypes , no significant signals were detected .
	manualset3
198747	6	416267	7	NULL	NULL	0	NULL	significant signals	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using statistical analyses for association of MCP3 polymorphisms with asthma development and asthma-related phenotypes , no significant signals were detected .
	manualset3
198748	1	416268	7	NULL	NULL	0	NULL	unsuccessful cardiopulmonary resuscitation efforts	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After unsuccessful cardiopulmonary resuscitation efforts , brain death was diagnosed .
	manualset3
198749	2	416268	7	NULL	NULL	0	NULL	brain death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After unsuccessful cardiopulmonary resuscitation efforts , brain death was diagnosed .
	manualset3
198750	1	416269	7	NULL	NULL	0	NULL	suitable assumptions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using suitable assumptions , we show the dynamic implications of the interaction between rational exemption , current and delayed information .
	manualset3
198751	2	416269	7	NULL	NULL	0	NULL	dynamic implications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using suitable assumptions , we show the dynamic implications of the interaction between rational exemption , current and delayed information .
	manualset3
198752	3	416269	7	NULL	NULL	0	NULL	interaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using suitable assumptions , we show the dynamic implications of the interaction between rational exemption , current and delayed information .
	manualset3
198753	4	416269	7	NULL	NULL	0	NULL	rational exemption 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using suitable assumptions , we show the dynamic implications of the interaction between rational exemption , current and delayed information .
	manualset3
198754	5	416269	7	NULL	NULL	0	NULL	 current information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Using suitable assumptions , we show the dynamic implications of the interaction between rational exemption , current and delayed information .
	manualset3
198755	6	416269	7	NULL	NULL	0	NULL	delayed information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Using suitable assumptions , we show the dynamic implications of the interaction between rational exemption , current and delayed information .
	manualset3
198756	1	416270	7	NULL	NULL	0	NULL	Clq-binding assay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the Clq-binding assay , circulating immune complexes were detected in mice given a single high dose of CP ( 466 microgram ) and repeated human-equivalent doses ( 70 microgram ) .
	manualset3
198757	2	416270	7	NULL	NULL	0	NULL	circulating immune complexes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the Clq-binding assay , circulating immune complexes were detected in mice given a single high dose of CP ( 466 microgram ) and repeated human-equivalent doses ( 70 microgram ) .
	manualset3
198758	3	416270	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the Clq-binding assay , circulating immune complexes were detected in mice given a single high dose of CP ( 466 microgram ) and repeated human-equivalent doses ( 70 microgram ) .
	manualset3
198759	4	416270	7	NULL	NULL	0	NULL	 single high dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the Clq-binding assay , circulating immune complexes were detected in mice given a single high dose of CP ( 466 microgram ) and repeated human-equivalent doses ( 70 microgram ) .
	manualset3
198760	5	416270	7	NULL	NULL	0	NULL	CP 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the Clq-binding assay , circulating immune complexes were detected in mice given a single high dose of CP ( 466 microgram ) and repeated human-equivalent doses ( 70 microgram ) .
	manualset3
198761	6	416270	7	NULL	NULL	0	NULL	466 microgram	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the Clq-binding assay , circulating immune complexes were detected in mice given a single high dose of CP ( 466 microgram ) and repeated human-equivalent doses ( 70 microgram ) .
	manualset3
198762	7	416270	7	NULL	NULL	0	NULL	human-equivalent doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the Clq-binding assay , circulating immune complexes were detected in mice given a single high dose of CP ( 466 microgram ) and repeated human-equivalent doses ( 70 microgram ) .
	manualset3
198763	8	416270	7	NULL	NULL	0	NULL	70 microgram 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the Clq-binding assay , circulating immune complexes were detected in mice given a single high dose of CP ( 466 microgram ) and repeated human-equivalent doses ( 70 microgram ) .
	manualset3
198764	1	416271	7	NULL	NULL	0	NULL	 DOCK methodology	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the DOCK methodology , we have carried out a structure-based , computer-assisted search of an available chemical database in order to identify low molecular weight , nonpeptidic PTP1B inhibitors .
	manualset3
198765	2	416271	7	NULL	NULL	0	NULL	structure-based , computer-assisted search	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the DOCK methodology , we have carried out a structure-based , computer-assisted search of an available chemical database in order to identify low molecular weight , nonpeptidic PTP1B inhibitors .
	manualset3
198766	3	416271	7	NULL	NULL	0	NULL	chemical database	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the DOCK methodology , we have carried out a structure-based , computer-assisted search of an available chemical database in order to identify low molecular weight , nonpeptidic PTP1B inhibitors .
	manualset3
198767	4	416271	7	NULL	NULL	0	NULL	low molecular weight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the DOCK methodology , we have carried out a structure-based , computer-assisted search of an available chemical database in order to identify low molecular weight , nonpeptidic PTP1B inhibitors .
	manualset3
198768	5	416271	7	NULL	NULL	0	NULL	nonpeptidic PTP1B inhibitors 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the DOCK methodology , we have carried out a structure-based , computer-assisted search of an available chemical database in order to identify low molecular weight , nonpeptidic PTP1B inhibitors .
	manualset3
198769	1	416272	7	NULL	NULL	0	NULL	MUSA system	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the MUSA system , it became easier to remove successfully tumorous mass and the nidus of AVM , because it minimized the risk of injury to the normal structures such as the surrounding brain tissue , vascular systems and the cranial nerves .
	manualset3
198770	2	416272	7	NULL	NULL	0	NULL	tumorous mass	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the MUSA system , it became easier to remove successfully tumorous mass and the nidus of AVM , because it minimized the risk of injury to the normal structures such as the surrounding brain tissue , vascular systems and the cranial nerves .
	manualset3
198771	3	416272	7	NULL	NULL	0	NULL	nidus of AVM	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the MUSA system , it became easier to remove successfully tumorous mass and the nidus of AVM , because it minimized the risk of injury to the normal structures such as the surrounding brain tissue , vascular systems and the cranial nerves .
	manualset3
198772	4	416272	7	NULL	NULL	0	NULL	 risk of injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the MUSA system , it became easier to remove successfully tumorous mass and the nidus of AVM , because it minimized the risk of injury to the normal structures such as the surrounding brain tissue , vascular systems and the cranial nerves .
	manualset3
198773	5	416272	7	NULL	NULL	0	NULL	normal structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the MUSA system , it became easier to remove successfully tumorous mass and the nidus of AVM , because it minimized the risk of injury to the normal structures such as the surrounding brain tissue , vascular systems and the cranial nerves .
	manualset3
198774	6	416272	7	NULL	NULL	0	NULL	brain tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the MUSA system , it became easier to remove successfully tumorous mass and the nidus of AVM , because it minimized the risk of injury to the normal structures such as the surrounding brain tissue , vascular systems and the cranial nerves .
	manualset3
198775	7	416272	7	NULL	NULL	0	NULL	vascular systems 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the MUSA system , it became easier to remove successfully tumorous mass and the nidus of AVM , because it minimized the risk of injury to the normal structures such as the surrounding brain tissue , vascular systems and the cranial nerves .
	manualset3
198776	8	416272	7	NULL	NULL	0	NULL	cranial nerves	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the MUSA system , it became easier to remove successfully tumorous mass and the nidus of AVM , because it minimized the risk of injury to the normal structures such as the surrounding brain tissue , vascular systems and the cranial nerves .
	manualset3
198777	1	416273	7	NULL	NULL	0	NULL	P19 embryonal cell line 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the P19 embryonal cell line , whole-cell current profiles of P19 cells before , during and after retinoic acid-induced differentiation were matched with their morphology as well as with the expression of neuron-specific enolase-like immunoreactivity .
	manualset3
198778	2	416273	7	NULL	NULL	0	NULL	whole-cell current profiles	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the P19 embryonal cell line , whole-cell current profiles of P19 cells before , during and after retinoic acid-induced differentiation were matched with their morphology as well as with the expression of neuron-specific enolase-like immunoreactivity .
	manualset3
198779	3	416273	7	NULL	NULL	0	NULL	P19 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the P19 embryonal cell line , whole-cell current profiles of P19 cells before , during and after retinoic acid-induced differentiation were matched with their morphology as well as with the expression of neuron-specific enolase-like immunoreactivity .
	manualset3
198780	4	416273	7	NULL	NULL	0	NULL	retinoic acid-induced differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the P19 embryonal cell line , whole-cell current profiles of P19 cells before , during and after retinoic acid-induced differentiation were matched with their morphology as well as with the expression of neuron-specific enolase-like immunoreactivity .
	manualset3
198781	5	416273	7	NULL	NULL	0	NULL	morphology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the P19 embryonal cell line , whole-cell current profiles of P19 cells before , during and after retinoic acid-induced differentiation were matched with their morphology as well as with the expression of neuron-specific enolase-like immunoreactivity .
	manualset3
198782	6	416273	7	NULL	NULL	0	NULL	expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the P19 embryonal cell line , whole-cell current profiles of P19 cells before , during and after retinoic acid-induced differentiation were matched with their morphology as well as with the expression of neuron-specific enolase-like immunoreactivity .
	manualset3
198783	7	416273	7	NULL	NULL	0	NULL	neuron-specific enolase-like immunoreactivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the P19 embryonal cell line , whole-cell current profiles of P19 cells before , during and after retinoic acid-induced differentiation were matched with their morphology as well as with the expression of neuron-specific enolase-like immunoreactivity .
	manualset3
198784	1	416274	7	NULL	NULL	0	NULL	THERdbASE exposure model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the THERdbASE exposure model and experimentally determined emission data , indoor air concentrations and daily intake values were determined for both types of rimblock products .
	manualset3
198785	2	416274	7	NULL	NULL	0	NULL	experimentally determined emission data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the THERdbASE exposure model and experimentally determined emission data , indoor air concentrations and daily intake values were determined for both types of rimblock products .
	manualset3
198786	3	416274	7	NULL	NULL	0	NULL	indoor air concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the THERdbASE exposure model and experimentally determined emission data , indoor air concentrations and daily intake values were determined for both types of rimblock products .
	manualset3
198787	4	416274	7	NULL	NULL	0	NULL	daily intake values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the THERdbASE exposure model and experimentally determined emission data , indoor air concentrations and daily intake values were determined for both types of rimblock products .
	manualset3
198788	5	416274	7	NULL	NULL	0	NULL	types	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the THERdbASE exposure model and experimentally determined emission data , indoor air concentrations and daily intake values were determined for both types of rimblock products .
	manualset3
198789	6	416274	7	NULL	NULL	0	NULL	rimblock products	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the THERdbASE exposure model and experimentally determined emission data , indoor air concentrations and daily intake values were determined for both types of rimblock products .
	manualset3
198790	1	416275	7	NULL	NULL	0	NULL	calcium-sensitive dye fura-2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the calcium-sensitive dye fura-2 , resting cytosolic free calcium concentrations ( ( Ca2 + ) i ) were found to be significantly higher in platelets of SHR compared to WKY ( 171.9 + / - 21.5 nmol/L v 93.14 + / - 19.7 nmol/L , P & lt ; .05 ) .
	manualset3
198791	2	416275	7	NULL	NULL	0	NULL	 resting cytosolic free calcium concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the calcium-sensitive dye fura-2 , resting cytosolic free calcium concentrations ( ( Ca2 + ) i ) were found to be significantly higher in platelets of SHR compared to WKY ( 171.9 + / - 21.5 nmol/L v 93.14 + / - 19.7 nmol/L , P & lt ; .05 ) .
	manualset3
198792	3	416275	7	NULL	NULL	0	NULL	( ( Ca2 + ) i )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the calcium-sensitive dye fura-2 , resting cytosolic free calcium concentrations ( ( Ca2 + ) i ) were found to be significantly higher in platelets of SHR compared to WKY ( 171.9 + / - 21.5 nmol/L v 93.14 + / - 19.7 nmol/L , P & lt ; .05 ) .
	manualset3
198793	4	416275	7	NULL	NULL	0	NULL	platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the calcium-sensitive dye fura-2 , resting cytosolic free calcium concentrations ( ( Ca2 + ) i ) were found to be significantly higher in platelets of SHR compared to WKY ( 171.9 + / - 21.5 nmol/L v 93.14 + / - 19.7 nmol/L , P & lt ; .05 ) .
	manualset3
198794	5	416275	7	NULL	NULL	0	NULL	SHR	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the calcium-sensitive dye fura-2 , resting cytosolic free calcium concentrations ( ( Ca2 + ) i ) were found to be significantly higher in platelets of SHR compared to WKY ( 171.9 + / - 21.5 nmol/L v 93.14 + / - 19.7 nmol/L , P & lt ; .05 ) .
	manualset3
198795	6	416275	7	NULL	NULL	0	NULL	WKY	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the calcium-sensitive dye fura-2 , resting cytosolic free calcium concentrations ( ( Ca2 + ) i ) were found to be significantly higher in platelets of SHR compared to WKY ( 171.9 + / - 21.5 nmol/L v 93.14 + / - 19.7 nmol/L , P & lt ; .05 ) .
	manualset3
198796	7	416275	7	NULL	NULL	0	NULL	171.9 + / - 21.5 nmol/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the calcium-sensitive dye fura-2 , resting cytosolic free calcium concentrations ( ( Ca2 + ) i ) were found to be significantly higher in platelets of SHR compared to WKY ( 171.9 + / - 21.5 nmol/L v 93.14 + / - 19.7 nmol/L , P & lt ; .05 ) .
	manualset3
198797	8	416275	7	NULL	NULL	0	NULL	93.14 + / - 19.7 nmol/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the calcium-sensitive dye fura-2 , resting cytosolic free calcium concentrations ( ( Ca2 + ) i ) were found to be significantly higher in platelets of SHR compared to WKY ( 171.9 + / - 21.5 nmol/L v 93.14 + / - 19.7 nmol/L , P & lt ; .05 ) .
	manualset3
198798	9	416275	7	NULL	NULL	0	NULL	 P & lt ; .05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the calcium-sensitive dye fura-2 , resting cytosolic free calcium concentrations ( ( Ca2 + ) i ) were found to be significantly higher in platelets of SHR compared to WKY ( 171.9 + / - 21.5 nmol/L v 93.14 + / - 19.7 nmol/L , P & lt ; .05 ) .
	manualset3
198799	1	416276	7	NULL	NULL	0	NULL	enzyme labeled ampicillin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the enzyme labeled ampicillin and anti-ampicillin serum , enzyme immunoassay of ampicillin was successful in detecting 4 ng to 1 mug .
	manualset3
198800	2	416276	7	NULL	NULL	0	NULL	anti-ampicillin serum	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the enzyme labeled ampicillin and anti-ampicillin serum , enzyme immunoassay of ampicillin was successful in detecting 4 ng to 1 mug .
	manualset3
198801	3	416276	7	NULL	NULL	0	NULL	enzyme immunoassay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the enzyme labeled ampicillin and anti-ampicillin serum , enzyme immunoassay of ampicillin was successful in detecting 4 ng to 1 mug .
	manualset3
198802	4	416276	7	NULL	NULL	0	NULL	ampicillin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the enzyme labeled ampicillin and anti-ampicillin serum , enzyme immunoassay of ampicillin was successful in detecting 4 ng to 1 mug .
	manualset3
198803	5	416276	7	NULL	NULL	0	NULL	detecting 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the enzyme labeled ampicillin and anti-ampicillin serum , enzyme immunoassay of ampicillin was successful in detecting 4 ng to 1 mug .
	manualset3
198804	6	416276	7	NULL	NULL	0	NULL	4 ng	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the enzyme labeled ampicillin and anti-ampicillin serum , enzyme immunoassay of ampicillin was successful in detecting 4 ng to 1 mug .
	manualset3
198805	7	416276	7	NULL	NULL	0	NULL	 1 mug	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the enzyme labeled ampicillin and anti-ampicillin serum , enzyme immunoassay of ampicillin was successful in detecting 4 ng to 1 mug .
	manualset3
198806	1	416277	7	NULL	NULL	NULL	NULL	 criteria	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using the former criteria , noradrenaline plus adrenaline ) 2.96 mmol l ( -1 ) , 1/15 in the phaeochromocytoma group had a normal result after clonidine suppression testing .
	manualset3
198807	2	416277	7	NULL	NULL	0	NULL	noradrenaline plus adrenaline )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the former criteria , noradrenaline plus adrenaline ) 2.96 mmol l ( -1 ) , 1/15 in the phaeochromocytoma group had a normal result after clonidine suppression testing .
	manualset3
198808	3	416277	7	NULL	NULL	0	NULL	2.96 mmol l ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the former criteria , noradrenaline plus adrenaline ) 2.96 mmol l ( -1 ) , 1/15 in the phaeochromocytoma group had a normal result after clonidine suppression testing .
	manualset3
198809	4	416277	7	NULL	NULL	0	NULL	1/15	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the former criteria , noradrenaline plus adrenaline ) 2.96 mmol l ( -1 ) , 1/15 in the phaeochromocytoma group had a normal result after clonidine suppression testing .
	manualset3
198810	5	416277	7	NULL	NULL	0	NULL	phaeochromocytoma group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the former criteria , noradrenaline plus adrenaline ) 2.96 mmol l ( -1 ) , 1/15 in the phaeochromocytoma group had a normal result after clonidine suppression testing .
	manualset3
198811	6	416277	7	NULL	NULL	0	NULL	normal result	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the former criteria , noradrenaline plus adrenaline ) 2.96 mmol l ( -1 ) , 1/15 in the phaeochromocytoma group had a normal result after clonidine suppression testing .
	manualset3
198812	7	416277	7	NULL	NULL	0	NULL	clonidine suppression testing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the former criteria , noradrenaline plus adrenaline ) 2.96 mmol l ( -1 ) , 1/15 in the phaeochromocytoma group had a normal result after clonidine suppression testing .
	manualset3
198813	1	416278	7	NULL	NULL	0	NULL	optimised method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the optimised method , 20 coffee and 15 chocolate samples collected from Valencian ( Spain ) supermarkets , were investigated for acrylamide , yielding median levels of 146 microg kg ( -1 ) in coffee and 102 microg kg ( -1 ) in chocolate .
	manualset3
198814	2	416278	7	NULL	NULL	NULL	NULL	20 coffee samples	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using the optimised method , 20 coffee and 15 chocolate samples collected from Valencian ( Spain ) supermarkets , were investigated for acrylamide , yielding median levels of 146 microg kg ( -1 ) in coffee and 102 microg kg ( -1 ) in chocolate .
	manualset3
198815	3	416278	7	NULL	NULL	NULL	NULL	15 chocolate samples	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using the optimised method , 20 coffee and 15 chocolate samples collected from Valencian ( Spain ) supermarkets , were investigated for acrylamide , yielding median levels of 146 microg kg ( -1 ) in coffee and 102 microg kg ( -1 ) in chocolate .
	manualset3
198816	4	416278	7	NULL	NULL	0	NULL	 Valencian ( Spain ) supermarkets	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the optimised method , 20 coffee and 15 chocolate samples collected from Valencian ( Spain ) supermarkets , were investigated for acrylamide , yielding median levels of 146 microg kg ( -1 ) in coffee and 102 microg kg ( -1 ) in chocolate .
	manualset3
198817	5	416278	7	NULL	NULL	0	NULL	acrylamide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the optimised method , 20 coffee and 15 chocolate samples collected from Valencian ( Spain ) supermarkets , were investigated for acrylamide , yielding median levels of 146 microg kg ( -1 ) in coffee and 102 microg kg ( -1 ) in chocolate .
	manualset3
198818	6	416278	7	NULL	NULL	0	NULL	median levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the optimised method , 20 coffee and 15 chocolate samples collected from Valencian ( Spain ) supermarkets , were investigated for acrylamide , yielding median levels of 146 microg kg ( -1 ) in coffee and 102 microg kg ( -1 ) in chocolate .
	manualset3
198819	7	416278	7	NULL	NULL	NULL	NULL	146 microg kg ( -1 )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using the optimised method , 20 coffee and 15 chocolate samples collected from Valencian ( Spain ) supermarkets , were investigated for acrylamide , yielding median levels of 146 microg kg ( -1 ) in coffee and 102 microg kg ( -1 ) in chocolate .
	manualset3
198820	8	416278	7	NULL	NULL	NULL	NULL	coffee	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using the optimised method , 20 coffee and 15 chocolate samples collected from Valencian ( Spain ) supermarkets , were investigated for acrylamide , yielding median levels of 146 microg kg ( -1 ) in coffee and 102 microg kg ( -1 ) in chocolate .
	manualset3
198821	9	416278	7	NULL	NULL	0	NULL	102 microg kg ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the optimised method , 20 coffee and 15 chocolate samples collected from Valencian ( Spain ) supermarkets , were investigated for acrylamide , yielding median levels of 146 microg kg ( -1 ) in coffee and 102 microg kg ( -1 ) in chocolate .
	manualset3
198822	10	416278	7	NULL	NULL	NULL	NULL	chocolate	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using the optimised method , 20 coffee and 15 chocolate samples collected from Valencian ( Spain ) supermarkets , were investigated for acrylamide , yielding median levels of 146 microg kg ( -1 ) in coffee and 102 microg kg ( -1 ) in chocolate .
	manualset3
198823	1	416279	7	NULL	NULL	0	NULL	patch-clamp technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the patch-clamp technique , we investigated Cl - channels on the basolateral membrane of the connecting tubule ( CNT ) and cortical collecting duct ( CCD ) .
	manualset3
198824	2	416279	7	NULL	NULL	0	NULL	Cl - channels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the patch-clamp technique , we investigated Cl - channels on the basolateral membrane of the connecting tubule ( CNT ) and cortical collecting duct ( CCD ) .
	manualset3
198825	3	416279	7	NULL	NULL	0	NULL	basolateral membrane	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the patch-clamp technique , we investigated Cl - channels on the basolateral membrane of the connecting tubule ( CNT ) and cortical collecting duct ( CCD ) .
	manualset3
198826	4	416279	7	NULL	NULL	0	NULL	connecting tubule ( CNT )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the patch-clamp technique , we investigated Cl - channels on the basolateral membrane of the connecting tubule ( CNT ) and cortical collecting duct ( CCD ) .
	manualset3
198827	5	416279	7	NULL	NULL	0	NULL	cortical collecting duct ( CCD )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the patch-clamp technique , we investigated Cl - channels on the basolateral membrane of the connecting tubule ( CNT ) and cortical collecting duct ( CCD ) .
	manualset3
198828	1	416280	7	NULL	NULL	0	NULL	principles	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the principles of participatory action research , data were collected from individual interviews , focus groups , and mail-out surveys of families who used the program .
	manualset3
198829	2	416280	7	NULL	NULL	0	NULL	participatory action research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the principles of participatory action research , data were collected from individual interviews , focus groups , and mail-out surveys of families who used the program .
	manualset3
198830	3	416280	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the principles of participatory action research , data were collected from individual interviews , focus groups , and mail-out surveys of families who used the program .
	manualset3
198831	4	416280	7	NULL	NULL	0	NULL	individual interviews	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the principles of participatory action research , data were collected from individual interviews , focus groups , and mail-out surveys of families who used the program .
	manualset3
198832	5	416280	7	NULL	NULL	0	NULL	 focus groups	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the principles of participatory action research , data were collected from individual interviews , focus groups , and mail-out surveys of families who used the program .
	manualset3
198833	6	416280	7	NULL	NULL	0	NULL	mail-out surveys	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the principles of participatory action research , data were collected from individual interviews , focus groups , and mail-out surveys of families who used the program .
	manualset3
198834	7	416280	7	NULL	NULL	0	NULL	families	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the principles of participatory action research , data were collected from individual interviews , focus groups , and mail-out surveys of families who used the program .
	manualset3
198835	8	416280	7	NULL	NULL	0	NULL	 program	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the principles of participatory action research , data were collected from individual interviews , focus groups , and mail-out surveys of families who used the program .
	manualset3
198836	1	416281	7	NULL	NULL	0	NULL	recombinant form	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the recombinant form of CDSN , either with its N-glycan chain or enzymatically deglycosylated , we also demonstrated that oligosaccharide residues do not protect CDSN against proteolysis by SCCE .
	manualset3
198837	2	416281	7	NULL	NULL	0	NULL	 CDSN	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the recombinant form of CDSN , either with its N-glycan chain or enzymatically deglycosylated , we also demonstrated that oligosaccharide residues do not protect CDSN against proteolysis by SCCE .
	manualset3
198838	3	416281	7	NULL	NULL	0	NULL	N-glycan chain	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the recombinant form of CDSN , either with its N-glycan chain or enzymatically deglycosylated , we also demonstrated that oligosaccharide residues do not protect CDSN against proteolysis by SCCE .
	manualset3
198839	4	416281	7	NULL	NULL	0	NULL	enzymatically deglycosylated 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the recombinant form of CDSN , either with its N-glycan chain or enzymatically deglycosylated , we also demonstrated that oligosaccharide residues do not protect CDSN against proteolysis by SCCE .
	manualset3
198840	5	416281	7	NULL	NULL	0	NULL	oligosaccharide residues	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the recombinant form of CDSN , either with its N-glycan chain or enzymatically deglycosylated , we also demonstrated that oligosaccharide residues do not protect CDSN against proteolysis by SCCE .
	manualset3
198841	6	416281	7	NULL	NULL	0	NULL	CDSN	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the recombinant form of CDSN , either with its N-glycan chain or enzymatically deglycosylated , we also demonstrated that oligosaccharide residues do not protect CDSN against proteolysis by SCCE .
	manualset3
198842	7	416281	7	NULL	NULL	0	NULL	proteolysis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the recombinant form of CDSN , either with its N-glycan chain or enzymatically deglycosylated , we also demonstrated that oligosaccharide residues do not protect CDSN against proteolysis by SCCE .
	manualset3
198843	8	416281	7	NULL	NULL	0	NULL	SCCE	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the recombinant form of CDSN , either with its N-glycan chain or enzymatically deglycosylated , we also demonstrated that oligosaccharide residues do not protect CDSN against proteolysis by SCCE .
	manualset3
198844	1	416282	7	NULL	NULL	0	NULL	replication-deficient adenovirus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the replication-deficient adenovirus , Ad-dl312 , and a plasmid-based firefly luciferase gene as a reporter , we have optimized the uptake and expression of DNA in rat submandibular glands in vivo .
	manualset3
198845	2	416282	7	NULL	NULL	0	NULL	Ad-dl312	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the replication-deficient adenovirus , Ad-dl312 , and a plasmid-based firefly luciferase gene as a reporter , we have optimized the uptake and expression of DNA in rat submandibular glands in vivo .
	manualset3
198846	3	416282	7	NULL	NULL	0	NULL	plasmid-based firefly luciferase gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the replication-deficient adenovirus , Ad-dl312 , and a plasmid-based firefly luciferase gene as a reporter , we have optimized the uptake and expression of DNA in rat submandibular glands in vivo .
	manualset3
198847	4	416282	7	NULL	NULL	0	NULL	 reporter	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the replication-deficient adenovirus , Ad-dl312 , and a plasmid-based firefly luciferase gene as a reporter , we have optimized the uptake and expression of DNA in rat submandibular glands in vivo .
	manualset3
198848	5	416282	7	NULL	NULL	0	NULL	uptake	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the replication-deficient adenovirus , Ad-dl312 , and a plasmid-based firefly luciferase gene as a reporter , we have optimized the uptake and expression of DNA in rat submandibular glands in vivo .
	manualset3
198849	6	416282	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the replication-deficient adenovirus , Ad-dl312 , and a plasmid-based firefly luciferase gene as a reporter , we have optimized the uptake and expression of DNA in rat submandibular glands in vivo .
	manualset3
198850	7	416282	7	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the replication-deficient adenovirus , Ad-dl312 , and a plasmid-based firefly luciferase gene as a reporter , we have optimized the uptake and expression of DNA in rat submandibular glands in vivo .
	manualset3
198851	8	416282	7	NULL	NULL	0	NULL	rat submandibular glands	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the replication-deficient adenovirus , Ad-dl312 , and a plasmid-based firefly luciferase gene as a reporter , we have optimized the uptake and expression of DNA in rat submandibular glands in vivo .
	manualset3
198852	1	416283	7	NULL	NULL	0	NULL	assay system	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the same assay system , sporozoites derived from salivary glands did not reinvade the salivary glands after inoculation .
	manualset3
198853	2	416283	7	NULL	NULL	0	NULL	sporozoites	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the same assay system , sporozoites derived from salivary glands did not reinvade the salivary glands after inoculation .
	manualset3
198854	3	416283	7	NULL	NULL	0	NULL	salivary glands	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the same assay system , sporozoites derived from salivary glands did not reinvade the salivary glands after inoculation .
	manualset3
198855	4	416283	7	NULL	NULL	0	NULL	salivary glands	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the same assay system , sporozoites derived from salivary glands did not reinvade the salivary glands after inoculation .
	manualset3
198856	5	416283	7	NULL	NULL	0	NULL	inoculation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the same assay system , sporozoites derived from salivary glands did not reinvade the salivary glands after inoculation .
	manualset3
198857	1	416284	7	NULL	NULL	0	NULL	model for BSM	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the same model for BSM , a worker exposed to the current threshold limit value of 0.2 mg/m3 for 40 years will sustain a risk of 2.22 ( 1.56-3 .48 ) .
	manualset3
198858	2	416284	7	NULL	NULL	0	NULL	worker	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the same model for BSM , a worker exposed to the current threshold limit value of 0.2 mg/m3 for 40 years will sustain a risk of 2.22 ( 1.56-3 .48 ) .
	manualset3
198859	3	416284	7	NULL	NULL	0	NULL	current threshold limit value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the same model for BSM , a worker exposed to the current threshold limit value of 0.2 mg/m3 for 40 years will sustain a risk of 2.22 ( 1.56-3 .48 ) .
	manualset3
198860	4	416284	7	NULL	NULL	0	NULL	 0.2 mg/m3	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the same model for BSM , a worker exposed to the current threshold limit value of 0.2 mg/m3 for 40 years will sustain a risk of 2.22 ( 1.56-3 .48 ) .
	manualset3
198861	5	416284	7	NULL	NULL	0	NULL	 40 years	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the same model for BSM , a worker exposed to the current threshold limit value of 0.2 mg/m3 for 40 years will sustain a risk of 2.22 ( 1.56-3 .48 ) .
	manualset3
198862	6	416284	7	NULL	NULL	0	NULL	 risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the same model for BSM , a worker exposed to the current threshold limit value of 0.2 mg/m3 for 40 years will sustain a risk of 2.22 ( 1.56-3 .48 ) .
	manualset3
198863	7	416284	7	NULL	NULL	0	NULL	2.22 ( 1.56-3 .48 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the same model for BSM , a worker exposed to the current threshold limit value of 0.2 mg/m3 for 40 years will sustain a risk of 2.22 ( 1.56-3 .48 ) .
	manualset3
198940	1	416285	7	NULL	NULL	0	NULL	 transgenic tobacco	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the transgenic tobacco expressing an apoprotein of Ca ( 2 + ) - sensitive photoprotein aequorin , evidence was obtained that cyclic mononucleotides ( cGMP , cAMP ) control the Ca2 + concentration in the cytoplasm testifying a crosstalk among Ca2 + and cyclic mononucleotides as messengers .
	manualset3
198941	2	416285	7	NULL	NULL	0	NULL	apoprotein of Ca ( 2 + ) - sensitive photoprotein aequorin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the transgenic tobacco expressing an apoprotein of Ca ( 2 + ) - sensitive photoprotein aequorin , evidence was obtained that cyclic mononucleotides ( cGMP , cAMP ) control the Ca2 + concentration in the cytoplasm testifying a crosstalk among Ca2 + and cyclic mononucleotides as messengers .
	manualset3
198942	3	416285	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the transgenic tobacco expressing an apoprotein of Ca ( 2 + ) - sensitive photoprotein aequorin , evidence was obtained that cyclic mononucleotides ( cGMP , cAMP ) control the Ca2 + concentration in the cytoplasm testifying a crosstalk among Ca2 + and cyclic mononucleotides as messengers .
	manualset3
198943	4	416285	7	NULL	NULL	0	NULL	cyclic mononucleotides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the transgenic tobacco expressing an apoprotein of Ca ( 2 + ) - sensitive photoprotein aequorin , evidence was obtained that cyclic mononucleotides ( cGMP , cAMP ) control the Ca2 + concentration in the cytoplasm testifying a crosstalk among Ca2 + and cyclic mononucleotides as messengers .
	manualset3
198944	5	416285	7	NULL	NULL	0	NULL	 cGMP	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the transgenic tobacco expressing an apoprotein of Ca ( 2 + ) - sensitive photoprotein aequorin , evidence was obtained that cyclic mononucleotides ( cGMP , cAMP ) control the Ca2 + concentration in the cytoplasm testifying a crosstalk among Ca2 + and cyclic mononucleotides as messengers .
	manualset3
198945	6	416285	7	NULL	NULL	0	NULL	cAMP	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the transgenic tobacco expressing an apoprotein of Ca ( 2 + ) - sensitive photoprotein aequorin , evidence was obtained that cyclic mononucleotides ( cGMP , cAMP ) control the Ca2 + concentration in the cytoplasm testifying a crosstalk among Ca2 + and cyclic mononucleotides as messengers .
	manualset3
198946	7	416285	7	NULL	NULL	0	NULL	Ca2 + concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the transgenic tobacco expressing an apoprotein of Ca ( 2 + ) - sensitive photoprotein aequorin , evidence was obtained that cyclic mononucleotides ( cGMP , cAMP ) control the Ca2 + concentration in the cytoplasm testifying a crosstalk among Ca2 + and cyclic mononucleotides as messengers .
	manualset3
198947	8	416285	7	NULL	NULL	0	NULL	cytoplasm	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the transgenic tobacco expressing an apoprotein of Ca ( 2 + ) - sensitive photoprotein aequorin , evidence was obtained that cyclic mononucleotides ( cGMP , cAMP ) control the Ca2 + concentration in the cytoplasm testifying a crosstalk among Ca2 + and cyclic mononucleotides as messengers .
	manualset3
198948	9	416285	7	NULL	NULL	0	NULL	 crosstalk	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the transgenic tobacco expressing an apoprotein of Ca ( 2 + ) - sensitive photoprotein aequorin , evidence was obtained that cyclic mononucleotides ( cGMP , cAMP ) control the Ca2 + concentration in the cytoplasm testifying a crosstalk among Ca2 + and cyclic mononucleotides as messengers .
	manualset3
198949	10	416285	7	NULL	NULL	0	NULL	Ca2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the transgenic tobacco expressing an apoprotein of Ca ( 2 + ) - sensitive photoprotein aequorin , evidence was obtained that cyclic mononucleotides ( cGMP , cAMP ) control the Ca2 + concentration in the cytoplasm testifying a crosstalk among Ca2 + and cyclic mononucleotides as messengers .
	manualset3
198950	11	416285	7	NULL	NULL	0	NULL	 cyclic mononucleotides 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the transgenic tobacco expressing an apoprotein of Ca ( 2 + ) - sensitive photoprotein aequorin , evidence was obtained that cyclic mononucleotides ( cGMP , cAMP ) control the Ca2 + concentration in the cytoplasm testifying a crosstalk among Ca2 + and cyclic mononucleotides as messengers .
	manualset3
198951	12	416285	7	NULL	NULL	0	NULL	messengers	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the transgenic tobacco expressing an apoprotein of Ca ( 2 + ) - sensitive photoprotein aequorin , evidence was obtained that cyclic mononucleotides ( cGMP , cAMP ) control the Ca2 + concentration in the cytoplasm testifying a crosstalk among Ca2 + and cyclic mononucleotides as messengers .
	manualset3
198952	1	416286	7	NULL	NULL	0	NULL	whole-cell recording patch clamp technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the whole-cell recording patch clamp technique in clonal cultures of human muscle satellite cells ( SC ) , we studied a voltage-gated potassium current analogous to the delayed rectifier current ( IKdr ) described in adult human skeletal muscle .
	manualset3
198953	2	416286	7	NULL	NULL	0	NULL	 clonal cultures	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the whole-cell recording patch clamp technique in clonal cultures of human muscle satellite cells ( SC ) , we studied a voltage-gated potassium current analogous to the delayed rectifier current ( IKdr ) described in adult human skeletal muscle .
	manualset3
198954	3	416286	7	NULL	NULL	0	NULL	human muscle satellite cells ( SC )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the whole-cell recording patch clamp technique in clonal cultures of human muscle satellite cells ( SC ) , we studied a voltage-gated potassium current analogous to the delayed rectifier current ( IKdr ) described in adult human skeletal muscle .
	manualset3
198955	4	416286	7	NULL	NULL	0	NULL	voltage-gated potassium current 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the whole-cell recording patch clamp technique in clonal cultures of human muscle satellite cells ( SC ) , we studied a voltage-gated potassium current analogous to the delayed rectifier current ( IKdr ) described in adult human skeletal muscle .
	manualset3
198956	5	416286	7	NULL	NULL	0	NULL	delayed rectifier current ( IKdr ) 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the whole-cell recording patch clamp technique in clonal cultures of human muscle satellite cells ( SC ) , we studied a voltage-gated potassium current analogous to the delayed rectifier current ( IKdr ) described in adult human skeletal muscle .
	manualset3
198957	6	416286	7	NULL	NULL	0	NULL	adult human skeletal muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Using the whole-cell recording patch clamp technique in clonal cultures of human muscle satellite cells ( SC ) , we studied a voltage-gated potassium current analogous to the delayed rectifier current ( IKdr ) described in adult human skeletal muscle .
	manualset3
198958	1	416287	7	NULL	NULL	0	NULL	effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this effect , we have measured the enthalpy ( DeltaH ) of loop cleavage and insertion for plasminogen activator inhibitor 1 ( PAI-1 ) as -38 kcal/mol .
	manualset3
198959	2	416287	7	NULL	NULL	0	NULL	enthalpy ( DeltaH )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this effect , we have measured the enthalpy ( DeltaH ) of loop cleavage and insertion for plasminogen activator inhibitor 1 ( PAI-1 ) as -38 kcal/mol .
	manualset3
198960	3	416287	7	NULL	NULL	0	NULL	loop cleavage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this effect , we have measured the enthalpy ( DeltaH ) of loop cleavage and insertion for plasminogen activator inhibitor 1 ( PAI-1 ) as -38 kcal/mol .
	manualset3
198961	4	416287	7	NULL	NULL	0	NULL	 insertion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this effect , we have measured the enthalpy ( DeltaH ) of loop cleavage and insertion for plasminogen activator inhibitor 1 ( PAI-1 ) as -38 kcal/mol .
	manualset3
198962	5	416287	7	NULL	NULL	0	NULL	plasminogen activator inhibitor 1 ( PAI-1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this effect , we have measured the enthalpy ( DeltaH ) of loop cleavage and insertion for plasminogen activator inhibitor 1 ( PAI-1 ) as -38 kcal/mol .
	manualset3
198963	6	416287	7	NULL	NULL	0	NULL	-38 kcal/mol	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this effect , we have measured the enthalpy ( DeltaH ) of loop cleavage and insertion for plasminogen activator inhibitor 1 ( PAI-1 ) as -38 kcal/mol .
	manualset3
198964	1	416288	7	NULL	NULL	0	NULL	fragment	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this fragment as a probe , we identified a restriction fragment length polymorphism ( RFLP ) of the para-homologous sodium channel gene between susceptible and kdr-type resistant German cockroaches .
	manualset3
198965	2	416288	7	NULL	NULL	0	NULL	probe	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this fragment as a probe , we identified a restriction fragment length polymorphism ( RFLP ) of the para-homologous sodium channel gene between susceptible and kdr-type resistant German cockroaches .
	manualset3
198966	3	416288	7	NULL	NULL	0	NULL	restriction fragment length polymorphism ( RFLP )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this fragment as a probe , we identified a restriction fragment length polymorphism ( RFLP ) of the para-homologous sodium channel gene between susceptible and kdr-type resistant German cockroaches .
	manualset3
198967	4	416288	7	NULL	NULL	0	NULL	para-homologous sodium channel gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this fragment as a probe , we identified a restriction fragment length polymorphism ( RFLP ) of the para-homologous sodium channel gene between susceptible and kdr-type resistant German cockroaches .
	manualset3
198968	5	416288	7	NULL	NULL	0	NULL	susceptible German cockroaches	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this fragment as a probe , we identified a restriction fragment length polymorphism ( RFLP ) of the para-homologous sodium channel gene between susceptible and kdr-type resistant German cockroaches .
	manualset3
198969	6	416288	7	NULL	NULL	0	NULL	kdr-type resistant German cockroaches	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this fragment as a probe , we identified a restriction fragment length polymorphism ( RFLP ) of the para-homologous sodium channel gene between susceptible and kdr-type resistant German cockroaches .
	manualset3
198970	1	416289	7	NULL	NULL	0	NULL	phenomenon	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this phenomenon alone or in combination with positive contrasts , we demonstrated identification of white , red , and mixed clots on a mouse model of myocardial infarction and human blood .
	manualset3
198971	2	416289	7	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this phenomenon alone or in combination with positive contrasts , we demonstrated identification of white , red , and mixed clots on a mouse model of myocardial infarction and human blood .
	manualset3
198972	3	416289	7	NULL	NULL	0	NULL	positive contrasts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this phenomenon alone or in combination with positive contrasts , we demonstrated identification of white , red , and mixed clots on a mouse model of myocardial infarction and human blood .
	manualset3
198973	4	416289	7	NULL	NULL	0	NULL	identification 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this phenomenon alone or in combination with positive contrasts , we demonstrated identification of white , red , and mixed clots on a mouse model of myocardial infarction and human blood .
	manualset3
198974	5	416289	7	NULL	NULL	0	NULL	white clots	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this phenomenon alone or in combination with positive contrasts , we demonstrated identification of white , red , and mixed clots on a mouse model of myocardial infarction and human blood .
	manualset3
198975	6	416289	7	NULL	NULL	0	NULL	red clots	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this phenomenon alone or in combination with positive contrasts , we demonstrated identification of white , red , and mixed clots on a mouse model of myocardial infarction and human blood .
	manualset3
198976	7	416289	7	NULL	NULL	0	NULL	mixed clots	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this phenomenon alone or in combination with positive contrasts , we demonstrated identification of white , red , and mixed clots on a mouse model of myocardial infarction and human blood .
	manualset3
198977	8	416289	7	NULL	NULL	0	NULL	mouse model 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this phenomenon alone or in combination with positive contrasts , we demonstrated identification of white , red , and mixed clots on a mouse model of myocardial infarction and human blood .
	manualset3
198978	9	416289	7	NULL	NULL	NULL	NULL	 myocardial infarction	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using this phenomenon alone or in combination with positive contrasts , we demonstrated identification of white , red , and mixed clots on a mouse model of myocardial infarction and human blood .
	manualset3
198979	10	416289	7	NULL	NULL	0	NULL	human blood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this phenomenon alone or in combination with positive contrasts , we demonstrated identification of white , red , and mixed clots on a mouse model of myocardial infarction and human blood .
	manualset3
198980	1	416290	7	NULL	NULL	0	NULL	 relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this relationship , we predict the effect of vaccinations that boost baseline CSP or TRAP antibody titers .
	manualset3
198981	2	416290	7	NULL	NULL	0	NULL	 effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this relationship , we predict the effect of vaccinations that boost baseline CSP or TRAP antibody titers .
	manualset3
198982	3	416290	7	NULL	NULL	0	NULL	vaccinations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this relationship , we predict the effect of vaccinations that boost baseline CSP or TRAP antibody titers .
	manualset3
198983	4	416290	7	NULL	NULL	NULL	NULL	 baseline CSP titers	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using this relationship , we predict the effect of vaccinations that boost baseline CSP or TRAP antibody titers .
	manualset3
198984	5	416290	7	NULL	NULL	0	NULL	TRAP antibody titers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this relationship , we predict the effect of vaccinations that boost baseline CSP or TRAP antibody titers .
	manualset3
198985	1	416291	7	NULL	NULL	0	NULL	technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this technique , the study showed that cumulus cells are essential for oocytes to mature from MI to MII but exposure to cumulus cells must occur before MI .
	manualset3
198986	2	416291	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this technique , the study showed that cumulus cells are essential for oocytes to mature from MI to MII but exposure to cumulus cells must occur before MI .
	manualset3
198987	3	416291	7	NULL	NULL	0	NULL	cumulus cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this technique , the study showed that cumulus cells are essential for oocytes to mature from MI to MII but exposure to cumulus cells must occur before MI .
	manualset3
198988	4	416291	7	NULL	NULL	0	NULL	oocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this technique , the study showed that cumulus cells are essential for oocytes to mature from MI to MII but exposure to cumulus cells must occur before MI .
	manualset3
198990	6	416291	7	NULL	NULL	0	NULL	MI	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this technique , the study showed that cumulus cells are essential for oocytes to mature from MI to MII but exposure to cumulus cells must occur before MI .
	manualset3
198991	7	416291	7	NULL	NULL	0	NULL	MII 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this technique , the study showed that cumulus cells are essential for oocytes to mature from MI to MII but exposure to cumulus cells must occur before MI .
	manualset3
198992	8	416291	7	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this technique , the study showed that cumulus cells are essential for oocytes to mature from MI to MII but exposure to cumulus cells must occur before MI .
	manualset3
198993	9	416291	7	NULL	NULL	0	NULL	cumulus cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this technique , the study showed that cumulus cells are essential for oocytes to mature from MI to MII but exposure to cumulus cells must occur before MI .
	manualset3
198994	10	416291	7	NULL	NULL	0	NULL	MI	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using this technique , the study showed that cumulus cells are essential for oocytes to mature from MI to MII but exposure to cumulus cells must occur before MI .
	manualset3
198995	1	416292	7	NULL	NULL	0	NULL	three different variations 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using three different variations of the highly sensitive polymerase chain reaction ( PCR ) - based assays for the detection of reverse transcriptase ( RT ) activity , we have verified the retroviral origin of the retrovirus-like particles that are produced in very low amounts by the MS cell lines .
	manualset3
198996	2	416292	7	NULL	NULL	0	NULL	highly sensitive polymerase chain reaction ( PCR ) - based assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using three different variations of the highly sensitive polymerase chain reaction ( PCR ) - based assays for the detection of reverse transcriptase ( RT ) activity , we have verified the retroviral origin of the retrovirus-like particles that are produced in very low amounts by the MS cell lines .
	manualset3
198997	3	416292	7	NULL	NULL	NULL	NULL	detection	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using three different variations of the highly sensitive polymerase chain reaction ( PCR ) - based assays for the detection of reverse transcriptase ( RT ) activity , we have verified the retroviral origin of the retrovirus-like particles that are produced in very low amounts by the MS cell lines .
	manualset3
198998	4	416292	7	NULL	NULL	0	NULL	reverse transcriptase ( RT ) activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using three different variations of the highly sensitive polymerase chain reaction ( PCR ) - based assays for the detection of reverse transcriptase ( RT ) activity , we have verified the retroviral origin of the retrovirus-like particles that are produced in very low amounts by the MS cell lines .
	manualset3
198999	5	416292	7	NULL	NULL	0	NULL	retroviral origin	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Using three different variations of the highly sensitive polymerase chain reaction ( PCR ) - based assays for the detection of reverse transcriptase ( RT ) activity , we have verified the retroviral origin of the retrovirus-like particles that are produced in very low amounts by the MS cell lines .
	manualset3
199000	6	416292	7	NULL	NULL	0	NULL	retrovirus-like particles	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Using three different variations of the highly sensitive polymerase chain reaction ( PCR ) - based assays for the detection of reverse transcriptase ( RT ) activity , we have verified the retroviral origin of the retrovirus-like particles that are produced in very low amounts by the MS cell lines .
	manualset3
199001	7	416292	7	NULL	NULL	0	NULL	 very low amounts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using three different variations of the highly sensitive polymerase chain reaction ( PCR ) - based assays for the detection of reverse transcriptase ( RT ) activity , we have verified the retroviral origin of the retrovirus-like particles that are produced in very low amounts by the MS cell lines .
	manualset3
199002	8	416292	7	NULL	NULL	0	NULL	MS cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using three different variations of the highly sensitive polymerase chain reaction ( PCR ) - based assays for the detection of reverse transcriptase ( RT ) activity , we have verified the retroviral origin of the retrovirus-like particles that are produced in very low amounts by the MS cell lines .
	manualset3
199003	1	416293	7	NULL	NULL	0	NULL	time-resolved single-wavelength IR spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using time-resolved single-wavelength IR spectroscopy , we determined a lower limit of 10 ( 6 ) s ( -1 ) for the rate constant of release of ATP from pHP-caged ATP at pH 7.0 .
	manualset3
199004	2	416293	7	NULL	NULL	0	NULL	 lower limit	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using time-resolved single-wavelength IR spectroscopy , we determined a lower limit of 10 ( 6 ) s ( -1 ) for the rate constant of release of ATP from pHP-caged ATP at pH 7.0 .
	manualset3
199005	3	416293	7	NULL	NULL	0	NULL	 10 ( 6 ) s ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Using time-resolved single-wavelength IR spectroscopy , we determined a lower limit of 10 ( 6 ) s ( -1 ) for the rate constant of release of ATP from pHP-caged ATP at pH 7.0 .
	manualset3
199006	4	416293	7	NULL	NULL	0	NULL	 rate constant	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using time-resolved single-wavelength IR spectroscopy , we determined a lower limit of 10 ( 6 ) s ( -1 ) for the rate constant of release of ATP from pHP-caged ATP at pH 7.0 .
	manualset3
199007	5	416293	7	NULL	NULL	0	NULL	 release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using time-resolved single-wavelength IR spectroscopy , we determined a lower limit of 10 ( 6 ) s ( -1 ) for the rate constant of release of ATP from pHP-caged ATP at pH 7.0 .
	manualset3
199008	6	416293	7	NULL	NULL	0	NULL	ATP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using time-resolved single-wavelength IR spectroscopy , we determined a lower limit of 10 ( 6 ) s ( -1 ) for the rate constant of release of ATP from pHP-caged ATP at pH 7.0 .
	manualset3
199009	7	416293	7	NULL	NULL	0	NULL	 pHP-caged ATP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using time-resolved single-wavelength IR spectroscopy , we determined a lower limit of 10 ( 6 ) s ( -1 ) for the rate constant of release of ATP from pHP-caged ATP at pH 7.0 .
	manualset3
199010	8	416293	7	NULL	NULL	0	NULL	pH 7.0	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using time-resolved single-wavelength IR spectroscopy , we determined a lower limit of 10 ( 6 ) s ( -1 ) for the rate constant of release of ATP from pHP-caged ATP at pH 7.0 .
	manualset3
199011	1	416294	7	NULL	NULL	0	NULL	 transient transfections	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using transient transfections , we now demonstrate that increasing the length of the leader sequence to 67 nucleotides indeed completely abolishes translation initiation at the second start codon , and thus expression of the betaA1-crystallin protein .
	manualset3
199012	2	416294	7	NULL	NULL	0	NULL	 increasing	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using transient transfections , we now demonstrate that increasing the length of the leader sequence to 67 nucleotides indeed completely abolishes translation initiation at the second start codon , and thus expression of the betaA1-crystallin protein .
	manualset3
199013	3	416294	7	NULL	NULL	0	NULL	length 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using transient transfections , we now demonstrate that increasing the length of the leader sequence to 67 nucleotides indeed completely abolishes translation initiation at the second start codon , and thus expression of the betaA1-crystallin protein .
	manualset3
199014	4	416294	7	NULL	NULL	0	NULL	leader sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using transient transfections , we now demonstrate that increasing the length of the leader sequence to 67 nucleotides indeed completely abolishes translation initiation at the second start codon , and thus expression of the betaA1-crystallin protein .
	manualset3
199015	5	416294	7	NULL	NULL	0	NULL	67 nucleotides	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using transient transfections , we now demonstrate that increasing the length of the leader sequence to 67 nucleotides indeed completely abolishes translation initiation at the second start codon , and thus expression of the betaA1-crystallin protein .
	manualset3
199016	6	416294	7	NULL	NULL	0	NULL	translation initiation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using transient transfections , we now demonstrate that increasing the length of the leader sequence to 67 nucleotides indeed completely abolishes translation initiation at the second start codon , and thus expression of the betaA1-crystallin protein .
	manualset3
199017	7	416294	7	NULL	NULL	0	NULL	second start codon 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using transient transfections , we now demonstrate that increasing the length of the leader sequence to 67 nucleotides indeed completely abolishes translation initiation at the second start codon , and thus expression of the betaA1-crystallin protein .
	manualset3
199018	8	416294	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using transient transfections , we now demonstrate that increasing the length of the leader sequence to 67 nucleotides indeed completely abolishes translation initiation at the second start codon , and thus expression of the betaA1-crystallin protein .
	manualset3
199019	9	416294	7	NULL	NULL	0	NULL	betaA1-crystallin protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using transient transfections , we now demonstrate that increasing the length of the leader sequence to 67 nucleotides indeed completely abolishes translation initiation at the second start codon , and thus expression of the betaA1-crystallin protein .
	manualset3
199020	1	416295	7	NULL	NULL	0	NULL	whole-cell recordings	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using whole-cell recordings from a rat spinal slice preparation , we set out to determine the basis for prolonged EPSPs in tonic cells and the implications for signal processing .
	manualset3
199021	2	416295	7	NULL	NULL	0	NULL	 rat spinal slice preparation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Using whole-cell recordings from a rat spinal slice preparation , we set out to determine the basis for prolonged EPSPs in tonic cells and the implications for signal processing .
	manualset3
199022	3	416295	7	NULL	NULL	0	NULL	basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using whole-cell recordings from a rat spinal slice preparation , we set out to determine the basis for prolonged EPSPs in tonic cells and the implications for signal processing .
	manualset3
199023	4	416295	7	NULL	NULL	0	NULL	 prolonged EPSPs 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using whole-cell recordings from a rat spinal slice preparation , we set out to determine the basis for prolonged EPSPs in tonic cells and the implications for signal processing .
	manualset3
199024	5	416295	7	NULL	NULL	0	NULL	tonic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using whole-cell recordings from a rat spinal slice preparation , we set out to determine the basis for prolonged EPSPs in tonic cells and the implications for signal processing .
	manualset3
199025	6	416295	7	NULL	NULL	NULL	NULL	implications 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using whole-cell recordings from a rat spinal slice preparation , we set out to determine the basis for prolonged EPSPs in tonic cells and the implications for signal processing .
	manualset3
199026	7	416295	7	NULL	NULL	0	NULL	signal processing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using whole-cell recordings from a rat spinal slice preparation , we set out to determine the basis for prolonged EPSPs in tonic cells and the implications for signal processing .
	manualset3
199027	1	416296	7	NULL	NULL	0	NULL	CGL	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Usually CGL is accompanied by the presence , in bone marrow cells , of the Ph chromosome , the first chromosomal anomaly to be regularly associated with a human neoplastic disease .
	manualset3
199028	2	416296	7	NULL	NULL	0	NULL	 presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Usually CGL is accompanied by the presence , in bone marrow cells , of the Ph chromosome , the first chromosomal anomaly to be regularly associated with a human neoplastic disease .
	manualset3
199029	3	416296	7	NULL	NULL	0	NULL	bone marrow cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Usually CGL is accompanied by the presence , in bone marrow cells , of the Ph chromosome , the first chromosomal anomaly to be regularly associated with a human neoplastic disease .
	manualset3
199030	4	416296	7	NULL	NULL	0	NULL	Ph chromosome	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Usually CGL is accompanied by the presence , in bone marrow cells , of the Ph chromosome , the first chromosomal anomaly to be regularly associated with a human neoplastic disease .
	manualset3
199031	5	416296	7	NULL	NULL	0	NULL	first chromosomal anomaly	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Usually CGL is accompanied by the presence , in bone marrow cells , of the Ph chromosome , the first chromosomal anomaly to be regularly associated with a human neoplastic disease .
	manualset3
199032	6	416296	7	NULL	NULL	0	NULL	human neoplastic disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Usually CGL is accompanied by the presence , in bone marrow cells , of the Ph chromosome , the first chromosomal anomaly to be regularly associated with a human neoplastic disease .
	manualset3
199033	1	416297	7	NULL	NULL	0	NULL	asymptomatic , splenosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Usually asymptomatic , splenosis is an incidental finding at surgery , unrelated to the splenosis , for intestinal obstruction or suspected appendicitis or gynaecological pathology .
	manualset3
199034	2	416297	7	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Usually asymptomatic , splenosis is an incidental finding at surgery , unrelated to the splenosis , for intestinal obstruction or suspected appendicitis or gynaecological pathology .
	manualset3
199035	3	416297	7	NULL	NULL	0	NULL	splenosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Usually asymptomatic , splenosis is an incidental finding at surgery , unrelated to the splenosis , for intestinal obstruction or suspected appendicitis or gynaecological pathology .
	manualset3
199036	4	416297	7	NULL	NULL	0	NULL	intestinal obstruction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Usually asymptomatic , splenosis is an incidental finding at surgery , unrelated to the splenosis , for intestinal obstruction or suspected appendicitis or gynaecological pathology .
	manualset3
199037	5	416297	7	NULL	NULL	0	NULL	suspected appendicitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Usually asymptomatic , splenosis is an incidental finding at surgery , unrelated to the splenosis , for intestinal obstruction or suspected appendicitis or gynaecological pathology .
	manualset3
199038	6	416297	7	NULL	NULL	0	NULL	gynaecological pathology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Usually asymptomatic , splenosis is an incidental finding at surgery , unrelated to the splenosis , for intestinal obstruction or suspected appendicitis or gynaecological pathology .
	manualset3
201570	7	416297	7	NULL	NULL	0	NULL	incidental finding 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Usually asymptomatic , splenosis is an incidental finding at surgery , unrelated to the splenosis , for intestinal obstruction or suspected appendicitis or gynaecological pathology .
	manualset3
199039	1	416298	7	NULL	NULL	0	NULL	 treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Usually only one treatment is needed , however , electrochemotherapy can be repeated several times every few weeks with equal effectiveness each time .
	manualset3
199040	2	416298	7	NULL	NULL	0	NULL	 electrochemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Usually only one treatment is needed , however , electrochemotherapy can be repeated several times every few weeks with equal effectiveness each time .
	manualset3
199041	3	416298	7	NULL	NULL	0	NULL	several times	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Usually only one treatment is needed , however , electrochemotherapy can be repeated several times every few weeks with equal effectiveness each time .
	manualset3
199042	4	416298	7	NULL	NULL	0	NULL	few weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Usually only one treatment is needed , however , electrochemotherapy can be repeated several times every few weeks with equal effectiveness each time .
	manualset3
199043	5	416298	7	NULL	NULL	0	NULL	equal effectiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Usually only one treatment is needed , however , electrochemotherapy can be repeated several times every few weeks with equal effectiveness each time .
	manualset3
199044	6	416298	7	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Usually only one treatment is needed , however , electrochemotherapy can be repeated several times every few weeks with equal effectiveness each time .
	manualset3
199045	1	416299	7	NULL	NULL	0	NULL	Uterine epithelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Uterine epithelial cells and blood vessel walls were positive for galectin-4 , while galectin-9 was detected predominantly in uterine epithelial cells and late gestational TGC .
	manualset3
199046	2	416299	7	NULL	NULL	0	NULL	blood vessel walls	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Uterine epithelial cells and blood vessel walls were positive for galectin-4 , while galectin-9 was detected predominantly in uterine epithelial cells and late gestational TGC .
	manualset3
199047	3	416299	7	NULL	NULL	NULL	NULL	galectin-4	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Uterine epithelial cells and blood vessel walls were positive for galectin-4 , while galectin-9 was detected predominantly in uterine epithelial cells and late gestational TGC .
	manualset3
199048	4	416299	7	NULL	NULL	NULL	NULL	galectin-9	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Uterine epithelial cells and blood vessel walls were positive for galectin-4 , while galectin-9 was detected predominantly in uterine epithelial cells and late gestational TGC .
	manualset3
199049	5	416299	7	NULL	NULL	0	NULL	 uterine epithelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Uterine epithelial cells and blood vessel walls were positive for galectin-4 , while galectin-9 was detected predominantly in uterine epithelial cells and late gestational TGC .
	manualset3
199050	6	416299	7	NULL	NULL	0	NULL	 late gestational TGC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Uterine epithelial cells and blood vessel walls were positive for galectin-4 , while galectin-9 was detected predominantly in uterine epithelial cells and late gestational TGC .
	manualset3
199051	1	416300	7	NULL	NULL	0	NULL	Uterine expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Uterine expression of vascular endothelial growth factor is increased by estradiol and tamoxifen .
	manualset3
199052	2	416300	7	NULL	NULL	0	NULL	vascular endothelial growth factor	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Uterine expression of vascular endothelial growth factor is increased by estradiol and tamoxifen .
	manualset3
199053	3	416300	7	NULL	NULL	0	NULL	estradiol 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Uterine expression of vascular endothelial growth factor is increased by estradiol and tamoxifen .
	manualset3
199054	4	416300	7	NULL	NULL	0	NULL	tamoxifen	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Uterine expression of vascular endothelial growth factor is increased by estradiol and tamoxifen .
	manualset3
199055	1	416301	7	NULL	NULL	NULL	NULL	Utility	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Utility of a herpes oncolytic virus for the detection of neural invasion by cancer .
	manualset3
199057	2	416301	7	NULL	NULL	0	NULL	herpes oncolytic virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Utility of a herpes oncolytic virus for the detection of neural invasion by cancer .
	manualset3
199058	3	416301	7	NULL	NULL	0	NULL	detection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Utility of a herpes oncolytic virus for the detection of neural invasion by cancer .
	manualset3
199059	4	416301	7	NULL	NULL	0	NULL	neural invasion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Utility of a herpes oncolytic virus for the detection of neural invasion by cancer .
	manualset3
199060	5	416301	7	NULL	NULL	0	NULL	cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Utility of a herpes oncolytic virus for the detection of neural invasion by cancer .
	manualset3
199061	1	416302	7	NULL	NULL	0	NULL	Triton WR1339 injections	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Utilizing Triton WR1339 injections , we found that the decrease in serum TG concentrations was associated with a marked fall in very low density lipoprotein secretion rate .
	manualset3
199062	2	416302	7	NULL	NULL	0	NULL	decrease	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Utilizing Triton WR1339 injections , we found that the decrease in serum TG concentrations was associated with a marked fall in very low density lipoprotein secretion rate .
	manualset3
199063	3	416302	7	NULL	NULL	0	NULL	serum TG concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Utilizing Triton WR1339 injections , we found that the decrease in serum TG concentrations was associated with a marked fall in very low density lipoprotein secretion rate .
	manualset3
199064	4	416302	7	NULL	NULL	0	NULL	marked fall 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Utilizing Triton WR1339 injections , we found that the decrease in serum TG concentrations was associated with a marked fall in very low density lipoprotein secretion rate .
	manualset3
199065	5	416302	7	NULL	NULL	0	NULL	very low density lipoprotein secretion rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Utilizing Triton WR1339 injections , we found that the decrease in serum TG concentrations was associated with a marked fall in very low density lipoprotein secretion rate .
	manualset3
199066	1	416303	7	NULL	NULL	0	NULL	Pseudomonas aeruginosa 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Against Pseudomonas aeruginosa , MICs of GR69153 and ceftazidime for 50 % of isolates tested ( MIC50s ) were , respectively , 1 and 2 micrograms/ml ; the corresponding MIC90s were 4 and 16 micrograms/ml .
	manualset3
199074	2	416303	7	NULL	NULL	0	NULL	MICs	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Against Pseudomonas aeruginosa , MICs of GR69153 and ceftazidime for 50 % of isolates tested ( MIC50s ) were , respectively , 1 and 2 micrograms/ml ; the corresponding MIC90s were 4 and 16 micrograms/ml .
	manualset3
199075	3	416303	7	NULL	NULL	0	NULL	GR69153	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Against Pseudomonas aeruginosa , MICs of GR69153 and ceftazidime for 50 % of isolates tested ( MIC50s ) were , respectively , 1 and 2 micrograms/ml ; the corresponding MIC90s were 4 and 16 micrograms/ml .
	manualset3
199076	4	416303	7	NULL	NULL	0	NULL	ceftazidime	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Against Pseudomonas aeruginosa , MICs of GR69153 and ceftazidime for 50 % of isolates tested ( MIC50s ) were , respectively , 1 and 2 micrograms/ml ; the corresponding MIC90s were 4 and 16 micrograms/ml .
	manualset3
199077	5	416303	7	NULL	NULL	0	NULL	50 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Against Pseudomonas aeruginosa , MICs of GR69153 and ceftazidime for 50 % of isolates tested ( MIC50s ) were , respectively , 1 and 2 micrograms/ml ; the corresponding MIC90s were 4 and 16 micrograms/ml .
	manualset3
199078	6	416303	7	NULL	NULL	0	NULL	isolates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Against Pseudomonas aeruginosa , MICs of GR69153 and ceftazidime for 50 % of isolates tested ( MIC50s ) were , respectively , 1 and 2 micrograms/ml ; the corresponding MIC90s were 4 and 16 micrograms/ml .
	manualset3
199079	7	416303	7	NULL	NULL	0	NULL	MIC50s	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Against Pseudomonas aeruginosa , MICs of GR69153 and ceftazidime for 50 % of isolates tested ( MIC50s ) were , respectively , 1 and 2 micrograms/ml ; the corresponding MIC90s were 4 and 16 micrograms/ml .
	manualset3
199080	8	416303	7	NULL	NULL	0	NULL	1  micrograms/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Against Pseudomonas aeruginosa , MICs of GR69153 and ceftazidime for 50 % of isolates tested ( MIC50s ) were , respectively , 1 and 2 micrograms/ml ; the corresponding MIC90s were 4 and 16 micrograms/ml .
	manualset3
199081	9	416303	7	NULL	NULL	0	NULL	 2 micrograms/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Against Pseudomonas aeruginosa , MICs of GR69153 and ceftazidime for 50 % of isolates tested ( MIC50s ) were , respectively , 1 and 2 micrograms/ml ; the corresponding MIC90s were 4 and 16 micrograms/ml .
	manualset3
199082	10	416303	7	NULL	NULL	0	NULL	MIC90s	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Against Pseudomonas aeruginosa , MICs of GR69153 and ceftazidime for 50 % of isolates tested ( MIC50s ) were , respectively , 1 and 2 micrograms/ml ; the corresponding MIC90s were 4 and 16 micrograms/ml .
	manualset3
199083	11	416303	7	NULL	NULL	0	NULL	4 micrograms/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Against Pseudomonas aeruginosa , MICs of GR69153 and ceftazidime for 50 % of isolates tested ( MIC50s ) were , respectively , 1 and 2 micrograms/ml ; the corresponding MIC90s were 4 and 16 micrograms/ml .
	manualset3
199084	12	416303	7	NULL	NULL	0	NULL	16 micrograms/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Against Pseudomonas aeruginosa , MICs of GR69153 and ceftazidime for 50 % of isolates tested ( MIC50s ) were , respectively , 1 and 2 micrograms/ml ; the corresponding MIC90s were 4 and 16 micrograms/ml .
	manualset3
199085	1	416304	7	NULL	NULL	NULL	NULL	balloon flotation catheter 	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Utilizing a balloon flotation catheter , we measured PVR at varying cardiac outputs .
	manualset3
199086	2	416304	7	NULL	NULL	0	NULL	PVR	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Utilizing a balloon flotation catheter , we measured PVR at varying cardiac outputs .
	manualset3
199087	3	416304	7	NULL	NULL	0	NULL	cardiac outputs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Utilizing a balloon flotation catheter , we measured PVR at varying cardiac outputs .
	manualset3
199088	1	416305	7	NULL	NULL	0	NULL	V-region mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	V-region mutation in vitro , in vivo , and in silico reveal the importance of the enzymatic properties of AID and the sequence environment .
	manualset3
199089	2	416305	7	NULL	NULL	0	NULL	enzymatic properties 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	V-region mutation in vitro , in vivo , and in silico reveal the importance of the enzymatic properties of AID and the sequence environment .
	manualset3
199090	3	416305	7	NULL	NULL	0	NULL	AID	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	V-region mutation in vitro , in vivo , and in silico reveal the importance of the enzymatic properties of AID and the sequence environment .
	manualset3
199091	4	416305	7	NULL	NULL	0	NULL	sequence environment 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	V-region mutation in vitro , in vivo , and in silico reveal the importance of the enzymatic properties of AID and the sequence environment .
	manualset3
199092	1	416306	7	NULL	NULL	0	NULL	DISTRIBUTION	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	V. DISTRIBUTION OF BLOOD GROUP ANTIGENS IN NAHUAS , YAQUIS , TARAHUMARAS , TARASCOS AND MIXTECOS .
	manualset3
199093	2	416306	7	NULL	NULL	0	NULL	BLOOD GROUP ANTIGENS	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	V. DISTRIBUTION OF BLOOD GROUP ANTIGENS IN NAHUAS , YAQUIS , TARAHUMARAS , TARASCOS AND MIXTECOS .
	manualset3
199094	3	416306	7	NULL	NULL	0	NULL	NAHUAS	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	V. DISTRIBUTION OF BLOOD GROUP ANTIGENS IN NAHUAS , YAQUIS , TARAHUMARAS , TARASCOS AND MIXTECOS .
	manualset3
199095	4	416306	7	NULL	NULL	0	NULL	YAQUIS	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	V. DISTRIBUTION OF BLOOD GROUP ANTIGENS IN NAHUAS , YAQUIS , TARAHUMARAS , TARASCOS AND MIXTECOS .
	manualset3
199096	5	416306	7	NULL	NULL	0	NULL	TARAHUMARAS	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	V. DISTRIBUTION OF BLOOD GROUP ANTIGENS IN NAHUAS , YAQUIS , TARAHUMARAS , TARASCOS AND MIXTECOS .
	manualset3
199097	6	416306	7	NULL	NULL	0	NULL	 TARASCOS	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	V. DISTRIBUTION OF BLOOD GROUP ANTIGENS IN NAHUAS , YAQUIS , TARAHUMARAS , TARASCOS AND MIXTECOS .
	manualset3
199098	7	416306	7	NULL	NULL	0	NULL	MIXTECOS	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	V. DISTRIBUTION OF BLOOD GROUP ANTIGENS IN NAHUAS , YAQUIS , TARAHUMARAS , TARASCOS AND MIXTECOS .
	manualset3
199099	1	416307	7	NULL	NULL	0	NULL	Differentiation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	V. Differentiation of drug sensitive - and resistant-strains by minimal inhibitory concentration of the drug and annual change of sensitivity of the bacteria to various drugs .
	manualset3
199100	2	416307	7	NULL	NULL	0	NULL	 drug sensitive -strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	V. Differentiation of drug sensitive - and resistant-strains by minimal inhibitory concentration of the drug and annual change of sensitivity of the bacteria to various drugs .
	manualset3
199101	3	416307	7	NULL	NULL	0	NULL	drug resistant-strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	V. Differentiation of drug sensitive - and resistant-strains by minimal inhibitory concentration of the drug and annual change of sensitivity of the bacteria to various drugs .
	manualset3
199102	4	416307	7	NULL	NULL	0	NULL	minimal inhibitory concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	V. Differentiation of drug sensitive - and resistant-strains by minimal inhibitory concentration of the drug and annual change of sensitivity of the bacteria to various drugs .
	manualset3
199103	5	416307	7	NULL	NULL	0	NULL	 drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	V. Differentiation of drug sensitive - and resistant-strains by minimal inhibitory concentration of the drug and annual change of sensitivity of the bacteria to various drugs .
	manualset3
199104	6	416307	7	NULL	NULL	0	NULL	 annual change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	V. Differentiation of drug sensitive - and resistant-strains by minimal inhibitory concentration of the drug and annual change of sensitivity of the bacteria to various drugs .
	manualset3
199105	7	416307	7	NULL	NULL	0	NULL	sensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	V. Differentiation of drug sensitive - and resistant-strains by minimal inhibitory concentration of the drug and annual change of sensitivity of the bacteria to various drugs .
	manualset3
199106	8	416307	7	NULL	NULL	0	NULL	 bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	V. Differentiation of drug sensitive - and resistant-strains by minimal inhibitory concentration of the drug and annual change of sensitivity of the bacteria to various drugs .
	manualset3
199107	9	416307	7	NULL	NULL	0	NULL	drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	V. Differentiation of drug sensitive - and resistant-strains by minimal inhibitory concentration of the drug and annual change of sensitivity of the bacteria to various drugs .
	manualset3
199108	1	416308	7	NULL	NULL	0	NULL	VEC MR measurements	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	VEC MR measurements of aortic and pulmonary flow provided left and right ventricular stroke volumes that correlated well with left ventricular stroke volumes determined by short-axis cine MR images ( r = .98 , SEE = 3.7 ml , and r = .95 , SEE = 4.8 ml , respectively ) .
	manualset3
199109	2	416308	7	NULL	NULL	0	NULL	aortic flow	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	VEC MR measurements of aortic and pulmonary flow provided left and right ventricular stroke volumes that correlated well with left ventricular stroke volumes determined by short-axis cine MR images ( r = .98 , SEE = 3.7 ml , and r = .95 , SEE = 4.8 ml , respectively ) .
	manualset3
199110	3	416308	7	NULL	NULL	0	NULL	pulmonary flow	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	VEC MR measurements of aortic and pulmonary flow provided left and right ventricular stroke volumes that correlated well with left ventricular stroke volumes determined by short-axis cine MR images ( r = .98 , SEE = 3.7 ml , and r = .95 , SEE = 4.8 ml , respectively ) .
	manualset3
199111	4	416308	7	NULL	NULL	0	NULL	left ventricular stroke volumes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	VEC MR measurements of aortic and pulmonary flow provided left and right ventricular stroke volumes that correlated well with left ventricular stroke volumes determined by short-axis cine MR images ( r = .98 , SEE = 3.7 ml , and r = .95 , SEE = 4.8 ml , respectively ) .
	manualset3
199112	5	416308	7	NULL	NULL	0	NULL	right ventricular stroke volumes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	VEC MR measurements of aortic and pulmonary flow provided left and right ventricular stroke volumes that correlated well with left ventricular stroke volumes determined by short-axis cine MR images ( r = .98 , SEE = 3.7 ml , and r = .95 , SEE = 4.8 ml , respectively ) .
	manualset3
199113	6	416308	7	NULL	NULL	NULL	NULL	left ventricular stroke volumes	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	VEC MR measurements of aortic and pulmonary flow provided left and right ventricular stroke volumes that correlated well with left ventricular stroke volumes determined by short-axis cine MR images ( r = .98 , SEE = 3.7 ml , and r = .95 , SEE = 4.8 ml , respectively ) .
	manualset3
199114	7	416308	7	NULL	NULL	0	NULL	short-axis cine MR images	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	VEC MR measurements of aortic and pulmonary flow provided left and right ventricular stroke volumes that correlated well with left ventricular stroke volumes determined by short-axis cine MR images ( r = .98 , SEE = 3.7 ml , and r = .95 , SEE = 4.8 ml , respectively ) .
	manualset3
199115	8	416308	7	NULL	NULL	0	NULL	 r = .98	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	VEC MR measurements of aortic and pulmonary flow provided left and right ventricular stroke volumes that correlated well with left ventricular stroke volumes determined by short-axis cine MR images ( r = .98 , SEE = 3.7 ml , and r = .95 , SEE = 4.8 ml , respectively ) .
	manualset3
199116	9	416308	7	NULL	NULL	0	NULL	SEE = 3.7 ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	VEC MR measurements of aortic and pulmonary flow provided left and right ventricular stroke volumes that correlated well with left ventricular stroke volumes determined by short-axis cine MR images ( r = .98 , SEE = 3.7 ml , and r = .95 , SEE = 4.8 ml , respectively ) .
	manualset3
199117	10	416308	7	NULL	NULL	0	NULL	 r = .95	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	VEC MR measurements of aortic and pulmonary flow provided left and right ventricular stroke volumes that correlated well with left ventricular stroke volumes determined by short-axis cine MR images ( r = .98 , SEE = 3.7 ml , and r = .95 , SEE = 4.8 ml , respectively ) .
	manualset3
199118	11	416308	7	NULL	NULL	0	NULL	SEE = 4.8 ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	VEC MR measurements of aortic and pulmonary flow provided left and right ventricular stroke volumes that correlated well with left ventricular stroke volumes determined by short-axis cine MR images ( r = .98 , SEE = 3.7 ml , and r = .95 , SEE = 4.8 ml , respectively ) .
	manualset3
199119	1	416309	7	NULL	NULL	0	NULL	VEGF-immunoreactive ( IR ) cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	VEGF-immunoreactive ( IR ) cells were detected in 40 of 83 tumors , mainly G cell and enterochromaffin cell neoplasms .
	manualset3
199120	2	416309	7	NULL	NULL	0	NULL	40 tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	VEGF-immunoreactive ( IR ) cells were detected in 40 of 83 tumors , mainly G cell and enterochromaffin cell neoplasms .
	manualset3
199121	3	416309	7	NULL	NULL	0	NULL	83 tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	VEGF-immunoreactive ( IR ) cells were detected in 40 of 83 tumors , mainly G cell and enterochromaffin cell neoplasms .
	manualset3
199122	4	416309	7	NULL	NULL	0	NULL	 G cell 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	VEGF-immunoreactive ( IR ) cells were detected in 40 of 83 tumors , mainly G cell and enterochromaffin cell neoplasms .
	manualset3
199123	5	416309	7	NULL	NULL	0	NULL	enterochromaffin cell neoplasms	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	VEGF-immunoreactive ( IR ) cells were detected in 40 of 83 tumors , mainly G cell and enterochromaffin cell neoplasms .
	manualset3
199124	1	416310	7	NULL	NULL	0	NULL	VEGF-induced vasculogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	VEGF-induced vasculogenesis and sprouting angiogenesis were rescued in transduced ES cultures differentiating in vitro as EBs .
	manualset3
199125	2	416310	7	NULL	NULL	0	NULL	sprouting angiogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	VEGF-induced vasculogenesis and sprouting angiogenesis were rescued in transduced ES cultures differentiating in vitro as EBs .
	manualset3
199126	3	416310	7	NULL	NULL	0	NULL	 transduced ES cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	VEGF-induced vasculogenesis and sprouting angiogenesis were rescued in transduced ES cultures differentiating in vitro as EBs .
	manualset3
199155	5	416310	7	NULL	NULL	NULL	NULL	 EBs	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	VEGF-induced vasculogenesis and sprouting angiogenesis were rescued in transduced ES cultures differentiating in vitro as EBs .
	manualset3
199156	4	416310	7	NULL	NULL	0	NULL	differentiating	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	VEGF-induced vasculogenesis and sprouting angiogenesis were rescued in transduced ES cultures differentiating in vitro as EBs .
	manualset3
199157	1	416311	7	NULL	NULL	0	NULL	Agarose gel electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Agarose and denaturing polyacrylamide gel electrophoresis were used to assess the DNA cleavage activities .
	manualset3
199158	2	416311	7	NULL	NULL	0	NULL	denaturing polyacrylamide gel electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Agarose and denaturing polyacrylamide gel electrophoresis were used to assess the DNA cleavage activities .
	manualset3
199159	3	416311	7	NULL	NULL	0	NULL	DNA cleavage activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Agarose and denaturing polyacrylamide gel electrophoresis were used to assess the DNA cleavage activities .
	manualset3
199160	1	416312	7	NULL	NULL	0	NULL	VF	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	VF occurred in 28 % ( 9/32 of the dogs ) during the first sequence , and the incidence was higher in the subgroups with maximal alternans ) or = 20 ms ( p & lt ; 0.05 ) , maximal shortening rate ) or = 30 % , and afterdepolarizations .
	manualset3
199161	2	416312	7	NULL	NULL	0	NULL	28 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	VF occurred in 28 % ( 9/32 of the dogs ) during the first sequence , and the incidence was higher in the subgroups with maximal alternans ) or = 20 ms ( p & lt ; 0.05 ) , maximal shortening rate ) or = 30 % , and afterdepolarizations .
	manualset3
199162	3	416312	7	NULL	NULL	0	NULL	9/32	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	VF occurred in 28 % ( 9/32 of the dogs ) during the first sequence , and the incidence was higher in the subgroups with maximal alternans ) or = 20 ms ( p & lt ; 0.05 ) , maximal shortening rate ) or = 30 % , and afterdepolarizations .
	manualset3
199164	4	416312	7	NULL	NULL	0	NULL	 dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	VF occurred in 28 % ( 9/32 of the dogs ) during the first sequence , and the incidence was higher in the subgroups with maximal alternans ) or = 20 ms ( p & lt ; 0.05 ) , maximal shortening rate ) or = 30 % , and afterdepolarizations .
	manualset3
199167	5	416312	7	NULL	NULL	NULL	NULL	first sequence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	VF occurred in 28 % ( 9/32 of the dogs ) during the first sequence , and the incidence was higher in the subgroups with maximal alternans ) or = 20 ms ( p & lt ; 0.05 ) , maximal shortening rate ) or = 30 % , and afterdepolarizations .
	manualset3
199168	6	416312	7	NULL	NULL	0	NULL	incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	VF occurred in 28 % ( 9/32 of the dogs ) during the first sequence , and the incidence was higher in the subgroups with maximal alternans ) or = 20 ms ( p & lt ; 0.05 ) , maximal shortening rate ) or = 30 % , and afterdepolarizations .
	manualset3
199171	7	416312	7	NULL	NULL	0	NULL	subgroups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	VF occurred in 28 % ( 9/32 of the dogs ) during the first sequence , and the incidence was higher in the subgroups with maximal alternans ) or = 20 ms ( p & lt ; 0.05 ) , maximal shortening rate ) or = 30 % , and afterdepolarizations .
	manualset3
199173	8	416312	7	NULL	NULL	0	NULL	maximal alternans	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	VF occurred in 28 % ( 9/32 of the dogs ) during the first sequence , and the incidence was higher in the subgroups with maximal alternans ) or = 20 ms ( p & lt ; 0.05 ) , maximal shortening rate ) or = 30 % , and afterdepolarizations .
	manualset3
199175	9	416312	7	NULL	NULL	0	NULL	20 ms	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	VF occurred in 28 % ( 9/32 of the dogs ) during the first sequence , and the incidence was higher in the subgroups with maximal alternans ) or = 20 ms ( p & lt ; 0.05 ) , maximal shortening rate ) or = 30 % , and afterdepolarizations .
	manualset3
199177	10	416312	7	NULL	NULL	0	NULL	p & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	VF occurred in 28 % ( 9/32 of the dogs ) during the first sequence , and the incidence was higher in the subgroups with maximal alternans ) or = 20 ms ( p & lt ; 0.05 ) , maximal shortening rate ) or = 30 % , and afterdepolarizations .
	manualset3
199178	11	416312	7	NULL	NULL	0	NULL	maximal shortening rate 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	VF occurred in 28 % ( 9/32 of the dogs ) during the first sequence , and the incidence was higher in the subgroups with maximal alternans ) or = 20 ms ( p & lt ; 0.05 ) , maximal shortening rate ) or = 30 % , and afterdepolarizations .
	manualset3
199179	12	416312	7	NULL	NULL	0	NULL	30 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	VF occurred in 28 % ( 9/32 of the dogs ) during the first sequence , and the incidence was higher in the subgroups with maximal alternans ) or = 20 ms ( p & lt ; 0.05 ) , maximal shortening rate ) or = 30 % , and afterdepolarizations .
	manualset3
199180	13	416312	7	NULL	NULL	0	NULL	afterdepolarizations	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	VF occurred in 28 % ( 9/32 of the dogs ) during the first sequence , and the incidence was higher in the subgroups with maximal alternans ) or = 20 ms ( p & lt ; 0.05 ) , maximal shortening rate ) or = 30 % , and afterdepolarizations .
	manualset3
199226	1	416313	7	NULL	NULL	0	NULL	VH 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	VH correlate with pathology in the limbic system and more specifically the amygdale that is frequently affected in PD and DLB but relatively preserved in other forms of parkinsonism often misdiagnosed as PD .
	manualset3
199227	2	416313	7	NULL	NULL	0	NULL	pathology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	VH correlate with pathology in the limbic system and more specifically the amygdale that is frequently affected in PD and DLB but relatively preserved in other forms of parkinsonism often misdiagnosed as PD .
	manualset3
199228	3	416313	7	NULL	NULL	0	NULL	 limbic system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	VH correlate with pathology in the limbic system and more specifically the amygdale that is frequently affected in PD and DLB but relatively preserved in other forms of parkinsonism often misdiagnosed as PD .
	manualset3
199229	4	416313	7	NULL	NULL	0	NULL	amygdale	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	VH correlate with pathology in the limbic system and more specifically the amygdale that is frequently affected in PD and DLB but relatively preserved in other forms of parkinsonism often misdiagnosed as PD .
	manualset3
199230	5	416313	7	NULL	NULL	0	NULL	PD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	VH correlate with pathology in the limbic system and more specifically the amygdale that is frequently affected in PD and DLB but relatively preserved in other forms of parkinsonism often misdiagnosed as PD .
	manualset3
199231	6	416313	7	NULL	NULL	0	NULL	DLB	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	VH correlate with pathology in the limbic system and more specifically the amygdale that is frequently affected in PD and DLB but relatively preserved in other forms of parkinsonism often misdiagnosed as PD .
	manualset3
199232	7	416313	7	NULL	NULL	0	NULL	forms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	VH correlate with pathology in the limbic system and more specifically the amygdale that is frequently affected in PD and DLB but relatively preserved in other forms of parkinsonism often misdiagnosed as PD .
	manualset3
199233	8	416313	7	NULL	NULL	0	NULL	parkinsonism	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	VH correlate with pathology in the limbic system and more specifically the amygdale that is frequently affected in PD and DLB but relatively preserved in other forms of parkinsonism often misdiagnosed as PD .
	manualset3
199234	9	416313	7	NULL	NULL	0	NULL	PD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	VH correlate with pathology in the limbic system and more specifically the amygdale that is frequently affected in PD and DLB but relatively preserved in other forms of parkinsonism often misdiagnosed as PD .
	manualset3
199709	1	416314	7	NULL	NULL	0	NULL	Inhaled nitric oxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	VIII : Inhaled nitric oxide requires exogenous surfactant therapy in the lamb model of congenital diaphragmatic hernia .
	manualset3
199712	2	416314	7	NULL	NULL	0	NULL	exogenous surfactant therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	VIII : Inhaled nitric oxide requires exogenous surfactant therapy in the lamb model of congenital diaphragmatic hernia .
	manualset3
199714	3	416314	7	NULL	NULL	0	NULL	lamb model 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	VIII : Inhaled nitric oxide requires exogenous surfactant therapy in the lamb model of congenital diaphragmatic hernia .
	manualset3
199726	4	416314	7	NULL	NULL	0	NULL	congenital diaphragmatic hernia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	VIII : Inhaled nitric oxide requires exogenous surfactant therapy in the lamb model of congenital diaphragmatic hernia .
	manualset3
201618	5	416314	7	NULL	NULL	0	NULL	VIII	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	VIII : Inhaled nitric oxide requires exogenous surfactant therapy in the lamb model of congenital diaphragmatic hernia .
	manualset3
199728	1	416315	7	NULL	NULL	0	NULL	VLDL	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	VLDL retained their apo C-III and the apo C-III : TG ratio decreased as TG contents increased .
	manualset3
199735	2	416315	7	NULL	NULL	0	NULL	apo C-III 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	VLDL retained their apo C-III and the apo C-III : TG ratio decreased as TG contents increased .
	manualset3
199738	3	416315	7	NULL	NULL	0	NULL	 apo C-III : TG ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	VLDL retained their apo C-III and the apo C-III : TG ratio decreased as TG contents increased .
	manualset3
199739	4	416315	7	NULL	NULL	0	NULL	TG contents 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	VLDL retained their apo C-III and the apo C-III : TG ratio decreased as TG contents increased .
	manualset3
199837	1	416316	7	NULL	NULL	0	NULL	VT	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	VT , DI and DE at first increased , then VT and DI decreased , while DE remained augmented .
	manualset3
199840	2	416316	7	NULL	NULL	0	NULL	DI	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	VT , DI and DE at first increased , then VT and DI decreased , while DE remained augmented .
	manualset3
199843	3	416316	7	NULL	NULL	0	NULL	 DE	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	VT , DI and DE at first increased , then VT and DI decreased , while DE remained augmented .
	manualset3
199847	4	416316	7	NULL	NULL	0	NULL	VT	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	VT , DI and DE at first increased , then VT and DI decreased , while DE remained augmented .
	manualset3
199850	5	416316	7	NULL	NULL	0	NULL	 DI	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	VT , DI and DE at first increased , then VT and DI decreased , while DE remained augmented .
	manualset3
199853	6	416316	7	NULL	NULL	0	NULL	DE	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	VT , DI and DE at first increased , then VT and DI decreased , while DE remained augmented .
	manualset3
199859	1	416317	7	NULL	NULL	0	NULL	VX-148 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	VX-148 is a novel , uncompetitive IMPDH inhibitor with a K ( i ) value of 6 nM against IMPDH type II enzyme .
	manualset3
199860	2	416317	7	NULL	NULL	0	NULL	uncompetitive IMPDH inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	VX-148 is a novel , uncompetitive IMPDH inhibitor with a K ( i ) value of 6 nM against IMPDH type II enzyme .
	manualset3
199861	3	416317	7	NULL	NULL	0	NULL	K ( i ) value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	VX-148 is a novel , uncompetitive IMPDH inhibitor with a K ( i ) value of 6 nM against IMPDH type II enzyme .
	manualset3
199862	4	416317	7	NULL	NULL	0	NULL	6 nM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	VX-148 is a novel , uncompetitive IMPDH inhibitor with a K ( i ) value of 6 nM against IMPDH type II enzyme .
	manualset3
199863	5	416317	7	NULL	NULL	0	NULL	 IMPDH type II enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	VX-148 is a novel , uncompetitive IMPDH inhibitor with a K ( i ) value of 6 nM against IMPDH type II enzyme .
	manualset3
199873	1	416318	7	NULL	NULL	0	NULL	Vaccinia mature virus infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Vaccinia mature virus infection triggers the activation of phosphatidylinositol 3-kinase ( PI3K ) / Akt signaling , and the treatment of cells with inhibitors to block P13K activation reduces virus entry in an integrin 1-dependent manner , suggesting that integrin 1-mediates PI3K/Akt activation induced by vaccinia virus and that this signaling pathway is essential for virus endocytosis .
	manualset3
199874	2	416318	7	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Vaccinia mature virus infection triggers the activation of phosphatidylinositol 3-kinase ( PI3K ) / Akt signaling , and the treatment of cells with inhibitors to block P13K activation reduces virus entry in an integrin 1-dependent manner , suggesting that integrin 1-mediates PI3K/Akt activation induced by vaccinia virus and that this signaling pathway is essential for virus endocytosis .
	manualset3
199875	3	416318	7	NULL	NULL	0	NULL	phosphatidylinositol 3-kinase ( PI3K ) / Akt signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Vaccinia mature virus infection triggers the activation of phosphatidylinositol 3-kinase ( PI3K ) / Akt signaling , and the treatment of cells with inhibitors to block P13K activation reduces virus entry in an integrin 1-dependent manner , suggesting that integrin 1-mediates PI3K/Akt activation induced by vaccinia virus and that this signaling pathway is essential for virus endocytosis .
	manualset3
199876	4	416318	7	NULL	NULL	NULL	NULL	 treatment	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Vaccinia mature virus infection triggers the activation of phosphatidylinositol 3-kinase ( PI3K ) / Akt signaling , and the treatment of cells with inhibitors to block P13K activation reduces virus entry in an integrin 1-dependent manner , suggesting that integrin 1-mediates PI3K/Akt activation induced by vaccinia virus and that this signaling pathway is essential for virus endocytosis .
	manualset3
199877	5	416318	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Vaccinia mature virus infection triggers the activation of phosphatidylinositol 3-kinase ( PI3K ) / Akt signaling , and the treatment of cells with inhibitors to block P13K activation reduces virus entry in an integrin 1-dependent manner , suggesting that integrin 1-mediates PI3K/Akt activation induced by vaccinia virus and that this signaling pathway is essential for virus endocytosis .
	manualset3
199878	6	416318	7	NULL	NULL	0	NULL	inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Vaccinia mature virus infection triggers the activation of phosphatidylinositol 3-kinase ( PI3K ) / Akt signaling , and the treatment of cells with inhibitors to block P13K activation reduces virus entry in an integrin 1-dependent manner , suggesting that integrin 1-mediates PI3K/Akt activation induced by vaccinia virus and that this signaling pathway is essential for virus endocytosis .
	manualset3
199879	7	416318	7	NULL	NULL	0	NULL	P13K activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Vaccinia mature virus infection triggers the activation of phosphatidylinositol 3-kinase ( PI3K ) / Akt signaling , and the treatment of cells with inhibitors to block P13K activation reduces virus entry in an integrin 1-dependent manner , suggesting that integrin 1-mediates PI3K/Akt activation induced by vaccinia virus and that this signaling pathway is essential for virus endocytosis .
	manualset3
199880	8	416318	7	NULL	NULL	0	NULL	virus entry	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Vaccinia mature virus infection triggers the activation of phosphatidylinositol 3-kinase ( PI3K ) / Akt signaling , and the treatment of cells with inhibitors to block P13K activation reduces virus entry in an integrin 1-dependent manner , suggesting that integrin 1-mediates PI3K/Akt activation induced by vaccinia virus and that this signaling pathway is essential for virus endocytosis .
	manualset3
199881	9	416318	7	NULL	NULL	0	NULL	 integrin 1-dependent manner	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Vaccinia mature virus infection triggers the activation of phosphatidylinositol 3-kinase ( PI3K ) / Akt signaling , and the treatment of cells with inhibitors to block P13K activation reduces virus entry in an integrin 1-dependent manner , suggesting that integrin 1-mediates PI3K/Akt activation induced by vaccinia virus and that this signaling pathway is essential for virus endocytosis .
	manualset3
199882	10	416318	7	NULL	NULL	0	NULL	integrin 1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Vaccinia mature virus infection triggers the activation of phosphatidylinositol 3-kinase ( PI3K ) / Akt signaling , and the treatment of cells with inhibitors to block P13K activation reduces virus entry in an integrin 1-dependent manner , suggesting that integrin 1-mediates PI3K/Akt activation induced by vaccinia virus and that this signaling pathway is essential for virus endocytosis .
	manualset3
199883	11	416318	7	NULL	NULL	0	NULL	PI3K/Akt activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Vaccinia mature virus infection triggers the activation of phosphatidylinositol 3-kinase ( PI3K ) / Akt signaling , and the treatment of cells with inhibitors to block P13K activation reduces virus entry in an integrin 1-dependent manner , suggesting that integrin 1-mediates PI3K/Akt activation induced by vaccinia virus and that this signaling pathway is essential for virus endocytosis .
	manualset3
199884	12	416318	7	NULL	NULL	0	NULL	vaccinia virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Vaccinia mature virus infection triggers the activation of phosphatidylinositol 3-kinase ( PI3K ) / Akt signaling , and the treatment of cells with inhibitors to block P13K activation reduces virus entry in an integrin 1-dependent manner , suggesting that integrin 1-mediates PI3K/Akt activation induced by vaccinia virus and that this signaling pathway is essential for virus endocytosis .
	manualset3
199885	13	416318	7	NULL	NULL	0	NULL	signaling pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Vaccinia mature virus infection triggers the activation of phosphatidylinositol 3-kinase ( PI3K ) / Akt signaling , and the treatment of cells with inhibitors to block P13K activation reduces virus entry in an integrin 1-dependent manner , suggesting that integrin 1-mediates PI3K/Akt activation induced by vaccinia virus and that this signaling pathway is essential for virus endocytosis .
	manualset3
199886	14	416318	7	NULL	NULL	0	NULL	virus endocytosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Vaccinia mature virus infection triggers the activation of phosphatidylinositol 3-kinase ( PI3K ) / Akt signaling , and the treatment of cells with inhibitors to block P13K activation reduces virus entry in an integrin 1-dependent manner , suggesting that integrin 1-mediates PI3K/Akt activation induced by vaccinia virus and that this signaling pathway is essential for virus endocytosis .
	manualset3
200175	1	416319	7	NULL	NULL	0	NULL	Vacuolation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Vacuolation was not seen in imbibed dormant seeds , suggesting that vacuolation is associated with germination .
	manualset3
200176	2	416319	7	NULL	NULL	0	NULL	imbibed dormant seeds	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Vacuolation was not seen in imbibed dormant seeds , suggesting that vacuolation is associated with germination .
	manualset3
200177	3	416319	7	NULL	NULL	0	NULL	vacuolation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Vacuolation was not seen in imbibed dormant seeds , suggesting that vacuolation is associated with germination .
	manualset3
200178	4	416319	7	NULL	NULL	0	NULL	germination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Vacuolation was not seen in imbibed dormant seeds , suggesting that vacuolation is associated with germination .
	manualset3
200179	1	416320	7	NULL	NULL	NULL	NULL	Vacuum exposure holder	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Vacuum exposure holder for microradiography .
	manualset3
200180	2	416320	7	NULL	NULL	NULL	NULL	microradiography	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Vacuum exposure holder for microradiography .
	manualset3
200181	1	416321	7	NULL	NULL	0	NULL	Agarose gel electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Agarose gel electrophoresis of DNA extracted from IBDV-infected cells revealed the characteristic laddering pattern of DNA fragmentation , which was more intense in infected CEFs than in Vero cells .
	manualset3
200182	2	416321	7	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Agarose gel electrophoresis of DNA extracted from IBDV-infected cells revealed the characteristic laddering pattern of DNA fragmentation , which was more intense in infected CEFs than in Vero cells .
	manualset3
200183	3	416321	7	NULL	NULL	0	NULL	IBDV-infected cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Agarose gel electrophoresis of DNA extracted from IBDV-infected cells revealed the characteristic laddering pattern of DNA fragmentation , which was more intense in infected CEFs than in Vero cells .
	manualset3
200184	4	416321	7	NULL	NULL	0	NULL	 laddering pattern	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Agarose gel electrophoresis of DNA extracted from IBDV-infected cells revealed the characteristic laddering pattern of DNA fragmentation , which was more intense in infected CEFs than in Vero cells .
	manualset3
200185	5	416321	7	NULL	NULL	0	NULL	DNA fragmentation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Agarose gel electrophoresis of DNA extracted from IBDV-infected cells revealed the characteristic laddering pattern of DNA fragmentation , which was more intense in infected CEFs than in Vero cells .
	manualset3
200186	6	416321	7	NULL	NULL	0	NULL	infected CEFs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Agarose gel electrophoresis of DNA extracted from IBDV-infected cells revealed the characteristic laddering pattern of DNA fragmentation , which was more intense in infected CEFs than in Vero cells .
	manualset3
200187	7	416321	7	NULL	NULL	0	NULL	Vero cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Agarose gel electrophoresis of DNA extracted from IBDV-infected cells revealed the characteristic laddering pattern of DNA fragmentation , which was more intense in infected CEFs than in Vero cells .
	manualset3
200188	1	416322	7	NULL	NULL	0	NULL	Vaginal delivery	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Vaginal delivery of dicephalic parapagus conjoined twins : case report and literature review .
	manualset3
200189	2	416322	7	NULL	NULL	0	NULL	dicephalic parapagus conjoined twins	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Vaginal delivery of dicephalic parapagus conjoined twins : case report and literature review .
	manualset3
200190	3	416322	7	NULL	NULL	0	NULL	case report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Vaginal delivery of dicephalic parapagus conjoined twins : case report and literature review .
	manualset3
200191	4	416322	7	NULL	NULL	0	NULL	 literature review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Vaginal delivery of dicephalic parapagus conjoined twins : case report and literature review .
	manualset3
200192	1	416323	7	NULL	NULL	0	NULL	Vailulu'u Seamount 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Vailulu'u Seamount , Samoa : Life and death on an active submarine volcano .
	manualset3
200193	2	416323	7	NULL	NULL	0	NULL	Samoa	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Vailulu'u Seamount , Samoa : Life and death on an active submarine volcano .
	manualset3
200194	3	416323	7	NULL	NULL	0	NULL	Life	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Vailulu'u Seamount , Samoa : Life and death on an active submarine volcano .
	manualset3
200195	4	416323	7	NULL	NULL	0	NULL	death 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Vailulu'u Seamount , Samoa : Life and death on an active submarine volcano .
	manualset3
200196	5	416323	7	NULL	NULL	0	NULL	active submarine volcano	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Vailulu'u Seamount , Samoa : Life and death on an active submarine volcano .
	manualset3
200197	1	416324	7	NULL	NULL	0	NULL	Validation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Validation of a new box trainer-related tracking device : the TrEndo .
	manualset3
200198	2	416324	7	NULL	NULL	0	NULL	new box trainer-related tracking device	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Validation of a new box trainer-related tracking device : the TrEndo .
	manualset3
200199	3	416324	7	NULL	NULL	0	NULL	TrEndo	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Validation of a new box trainer-related tracking device : the TrEndo .
	manualset3
200200	1	416325	7	NULL	NULL	0	NULL	Validation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Validation of optical coherence tomography-based crystalline lens thickness measurements in children .
	manualset3
200201	2	416325	7	NULL	NULL	0	NULL	optical coherence tomography-based crystalline lens thickness measurements 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Validation of optical coherence tomography-based crystalline lens thickness measurements in children .
	manualset3
200202	3	416325	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Validation of optical coherence tomography-based crystalline lens thickness measurements in children .
	manualset3
200203	1	416326	7	NULL	NULL	0	NULL	Age-appropriate performance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Age-appropriate performance was also evident at kindergarten , except for lower math scores .
	manualset3
200204	2	416326	7	NULL	NULL	0	NULL	kindergarten	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Age-appropriate performance was also evident at kindergarten , except for lower math scores .
	manualset3
200205	3	416326	7	NULL	NULL	0	NULL	lower math scores	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Age-appropriate performance was also evident at kindergarten , except for lower math scores .
	manualset3
200206	1	416327	7	NULL	NULL	NULL	NULL	Validation	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Validation of the microarray for its sensitivity specificity and quantitation were performed using DNA isolated from well-characterized mixed bacterial cultures also having non-target strains , pure degrader strains , and environmental DNA .
	manualset3
200207	2	416327	7	NULL	NULL	0	NULL	microarray	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Validation of the microarray for its sensitivity specificity and quantitation were performed using DNA isolated from well-characterized mixed bacterial cultures also having non-target strains , pure degrader strains , and environmental DNA .
	manualset3
200208	3	416327	7	NULL	NULL	0	NULL	sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Validation of the microarray for its sensitivity specificity and quantitation were performed using DNA isolated from well-characterized mixed bacterial cultures also having non-target strains , pure degrader strains , and environmental DNA .
	manualset3
200209	4	416327	7	NULL	NULL	0	NULL	specificity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Validation of the microarray for its sensitivity specificity and quantitation were performed using DNA isolated from well-characterized mixed bacterial cultures also having non-target strains , pure degrader strains , and environmental DNA .
	manualset3
200210	5	416327	7	NULL	NULL	0	NULL	quantitation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Validation of the microarray for its sensitivity specificity and quantitation were performed using DNA isolated from well-characterized mixed bacterial cultures also having non-target strains , pure degrader strains , and environmental DNA .
	manualset3
200211	6	416327	7	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Validation of the microarray for its sensitivity specificity and quantitation were performed using DNA isolated from well-characterized mixed bacterial cultures also having non-target strains , pure degrader strains , and environmental DNA .
	manualset3
200212	7	416327	7	NULL	NULL	0	NULL	bacterial cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Validation of the microarray for its sensitivity specificity and quantitation were performed using DNA isolated from well-characterized mixed bacterial cultures also having non-target strains , pure degrader strains , and environmental DNA .
	manualset3
200213	8	416327	7	NULL	NULL	0	NULL	non-target strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Validation of the microarray for its sensitivity specificity and quantitation were performed using DNA isolated from well-characterized mixed bacterial cultures also having non-target strains , pure degrader strains , and environmental DNA .
	manualset3
200214	9	416327	7	NULL	NULL	0	NULL	pure degrader strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Validation of the microarray for its sensitivity specificity and quantitation were performed using DNA isolated from well-characterized mixed bacterial cultures also having non-target strains , pure degrader strains , and environmental DNA .
	manualset3
200215	10	416327	7	NULL	NULL	0	NULL	environmental DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Validation of the microarray for its sensitivity specificity and quantitation were performed using DNA isolated from well-characterized mixed bacterial cultures also having non-target strains , pure degrader strains , and environmental DNA .
	manualset3
200216	1	416328	7	NULL	NULL	0	NULL	Validity 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Validity of Demirjian 's and modified Demirjian 's methods in age estimation for Korean juveniles and adolescents .
	manualset3
200217	2	416328	7	NULL	NULL	0	NULL	Demirjian 's methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Validity of Demirjian 's and modified Demirjian 's methods in age estimation for Korean juveniles and adolescents .
	manualset3
200218	3	416328	7	NULL	NULL	0	NULL	modified Demirjian 's methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Validity of Demirjian 's and modified Demirjian 's methods in age estimation for Korean juveniles and adolescents .
	manualset3
200219	4	416328	7	NULL	NULL	0	NULL	age estimation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Validity of Demirjian 's and modified Demirjian 's methods in age estimation for Korean juveniles and adolescents .
	manualset3
200220	5	416328	7	NULL	NULL	0	NULL	Korean juveniles	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Validity of Demirjian 's and modified Demirjian 's methods in age estimation for Korean juveniles and adolescents .
	manualset3
200221	6	416328	7	NULL	NULL	0	NULL	adolescents 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Validity of Demirjian 's and modified Demirjian 's methods in age estimation for Korean juveniles and adolescents .
	manualset3
200222	1	416329	7	NULL	NULL	0	NULL	Validity	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Validity of Lot Quality Assurance Sampling to optimize falciparum malaria surveys in low-transmission areas .
	manualset3
200223	2	416329	7	NULL	NULL	0	NULL	Lot Quality Assurance Sampling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Validity of Lot Quality Assurance Sampling to optimize falciparum malaria surveys in low-transmission areas .
	manualset3
200224	3	416329	7	NULL	NULL	0	NULL	falciparum malaria surveys	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Validity of Lot Quality Assurance Sampling to optimize falciparum malaria surveys in low-transmission areas .
	manualset3
200225	4	416329	7	NULL	NULL	0	NULL	low-transmission areas 	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Validity of Lot Quality Assurance Sampling to optimize falciparum malaria surveys in low-transmission areas .
	manualset3
200226	1	416330	7	NULL	NULL	0	NULL	Validity	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Validity and reliability of qualitative dietary fat index questionnaires : a review .
	manualset3
200227	2	416330	7	NULL	NULL	0	NULL	reliability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Validity and reliability of qualitative dietary fat index questionnaires : a review .
	manualset3
200228	3	416330	7	NULL	NULL	0	NULL	 qualitative dietary fat index questionnaires	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Validity and reliability of qualitative dietary fat index questionnaires : a review .
	manualset3
200229	4	416330	7	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Validity and reliability of qualitative dietary fat index questionnaires : a review .
	manualset3
200286	1	417331	7	NULL	NULL	0	NULL	dipole-dipole interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We show that the dipole-dipole interactions between Rydberg excited atoms prevents the formation of single particle dark states and leads to strongly correlated photon pairs from atoms separated by distances large compared to the emission wavelength .
	manualset3
200287	2	417331	7	NULL	NULL	0	NULL	Rydberg excited atoms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We show that the dipole-dipole interactions between Rydberg excited atoms prevents the formation of single particle dark states and leads to strongly correlated photon pairs from atoms separated by distances large compared to the emission wavelength .
	manualset3
200288	3	417331	7	NULL	NULL	0	NULL	formation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We show that the dipole-dipole interactions between Rydberg excited atoms prevents the formation of single particle dark states and leads to strongly correlated photon pairs from atoms separated by distances large compared to the emission wavelength .
	manualset3
200289	4	417331	7	NULL	NULL	0	NULL	single particle dark states	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We show that the dipole-dipole interactions between Rydberg excited atoms prevents the formation of single particle dark states and leads to strongly correlated photon pairs from atoms separated by distances large compared to the emission wavelength .
	manualset3
200290	5	417331	7	NULL	NULL	0	NULL	photon pairs	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	We show that the dipole-dipole interactions between Rydberg excited atoms prevents the formation of single particle dark states and leads to strongly correlated photon pairs from atoms separated by distances large compared to the emission wavelength .
	manualset3
200291	6	417331	7	NULL	NULL	0	NULL	atoms 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	We show that the dipole-dipole interactions between Rydberg excited atoms prevents the formation of single particle dark states and leads to strongly correlated photon pairs from atoms separated by distances large compared to the emission wavelength .
	manualset3
200292	7	417331	7	NULL	NULL	0	NULL	distances	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We show that the dipole-dipole interactions between Rydberg excited atoms prevents the formation of single particle dark states and leads to strongly correlated photon pairs from atoms separated by distances large compared to the emission wavelength .
	manualset3
200293	8	417331	7	NULL	NULL	0	NULL	 emission wavelength	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We show that the dipole-dipole interactions between Rydberg excited atoms prevents the formation of single particle dark states and leads to strongly correlated photon pairs from atoms separated by distances large compared to the emission wavelength .
	manualset3
200294	1	417332	7	NULL	NULL	0	NULL	electronic structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We show that the electronic structure of compound Q can be understood as a dimer of two Fe ( IV ) O ( 2 + ) units .
	manualset3
200295	2	417332	7	NULL	NULL	0	NULL	compound Q	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We show that the electronic structure of compound Q can be understood as a dimer of two Fe ( IV ) O ( 2 + ) units .
	manualset3
200296	3	417332	7	NULL	NULL	0	NULL	dimer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We show that the electronic structure of compound Q can be understood as a dimer of two Fe ( IV ) O ( 2 + ) units .
	manualset3
200297	4	417332	7	NULL	NULL	0	NULL	two Fe ( IV ) O ( 2 + ) units	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We show that the electronic structure of compound Q can be understood as a dimer of two Fe ( IV ) O ( 2 + ) units .
	manualset3
200298	1	417333	7	NULL	NULL	0	NULL	structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We show that the structure of crystal quartz is not changed by repeated illumination of the focal region with 45 fs pulses .
	manualset3
200299	2	417333	7	NULL	NULL	0	NULL	crystal quartz	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We show that the structure of crystal quartz is not changed by repeated illumination of the focal region with 45 fs pulses .
	manualset3
200300	3	417333	7	NULL	NULL	0	NULL	repeated illumination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We show that the structure of crystal quartz is not changed by repeated illumination of the focal region with 45 fs pulses .
	manualset3
200301	4	417333	7	NULL	NULL	0	NULL	focal region	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We show that the structure of crystal quartz is not changed by repeated illumination of the focal region with 45 fs pulses .
	manualset3
200302	5	417333	7	NULL	NULL	0	NULL	45 fs pulses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We show that the structure of crystal quartz is not changed by repeated illumination of the focal region with 45 fs pulses .
	manualset3
200303	1	417334	7	NULL	NULL	0	NULL	three distinct chromatin proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We show that three distinct chromatin proteins in Drosophila melanogaster cells each associate with specific sets of genes .
	manualset3
200304	2	417334	7	NULL	NULL	0	NULL	Drosophila melanogaster cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We show that three distinct chromatin proteins in Drosophila melanogaster cells each associate with specific sets of genes .
	manualset3
200306	3	417334	7	NULL	NULL	0	NULL	specific sets 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We show that three distinct chromatin proteins in Drosophila melanogaster cells each associate with specific sets of genes .
	manualset3
200307	4	417334	7	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We show that three distinct chromatin proteins in Drosophila melanogaster cells each associate with specific sets of genes .
	manualset3
200308	1	417335	7	NULL	NULL	0	NULL	immunohistochemical study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed by immunohistochemical study that RIG-I expression is upregulated in vivo in hepatic Kupffer cells and in splenic reticular cells of mice infected with Listeria monocytogenes .
	manualset3
200309	2	417335	7	NULL	NULL	0	NULL	RIG-I expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed by immunohistochemical study that RIG-I expression is upregulated in vivo in hepatic Kupffer cells and in splenic reticular cells of mice infected with Listeria monocytogenes .
	manualset3
200310	3	417335	7	NULL	NULL	0	NULL	hepatic Kupffer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed by immunohistochemical study that RIG-I expression is upregulated in vivo in hepatic Kupffer cells and in splenic reticular cells of mice infected with Listeria monocytogenes .
	manualset3
200311	4	417335	7	NULL	NULL	0	NULL	splenic reticular cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed by immunohistochemical study that RIG-I expression is upregulated in vivo in hepatic Kupffer cells and in splenic reticular cells of mice infected with Listeria monocytogenes .
	manualset3
200312	5	417335	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed by immunohistochemical study that RIG-I expression is upregulated in vivo in hepatic Kupffer cells and in splenic reticular cells of mice infected with Listeria monocytogenes .
	manualset3
200313	6	417335	7	NULL	NULL	0	NULL	Listeria monocytogenes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed by immunohistochemical study that RIG-I expression is upregulated in vivo in hepatic Kupffer cells and in splenic reticular cells of mice infected with Listeria monocytogenes .
	manualset3
200314	1	417336	7	NULL	NULL	0	NULL	RepK 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed that RepK can bind to the fragment 13 but not to fragment 32 which lacks the 3 ' - moiety of fragment 13 .
	manualset3
200315	2	417336	7	NULL	NULL	0	NULL	fragment 13	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed that RepK can bind to the fragment 13 but not to fragment 32 which lacks the 3 ' - moiety of fragment 13 .
	manualset3
200316	3	417336	7	NULL	NULL	0	NULL	fragment 32	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed that RepK can bind to the fragment 13 but not to fragment 32 which lacks the 3 ' - moiety of fragment 13 .
	manualset3
200317	4	417336	7	NULL	NULL	0	NULL	 3 ' - moiety	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed that RepK can bind to the fragment 13 but not to fragment 32 which lacks the 3 ' - moiety of fragment 13 .
	manualset3
200318	5	417336	7	NULL	NULL	0	NULL	fragment 13	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed that RepK can bind to the fragment 13 but not to fragment 32 which lacks the 3 ' - moiety of fragment 13 .
	manualset3
200319	1	417337	7	NULL	NULL	0	NULL	 exposure	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed that exposure of Xenopus embryos to 0.5 % alcohol from stage 13 to stage 22 produced tadpoles with delayed gut maturation , reduced growth , and down-regulation in several gut developmental genes , with VegT , Pax6 and Sox17 most vulnerable .
	manualset3
200320	2	417337	7	NULL	NULL	0	NULL	Xenopus embryos	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed that exposure of Xenopus embryos to 0.5 % alcohol from stage 13 to stage 22 produced tadpoles with delayed gut maturation , reduced growth , and down-regulation in several gut developmental genes , with VegT , Pax6 and Sox17 most vulnerable .
	manualset3
200321	3	417337	7	NULL	NULL	0	NULL	0.5 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed that exposure of Xenopus embryos to 0.5 % alcohol from stage 13 to stage 22 produced tadpoles with delayed gut maturation , reduced growth , and down-regulation in several gut developmental genes , with VegT , Pax6 and Sox17 most vulnerable .
	manualset3
200322	4	417337	7	NULL	NULL	0	NULL	alcohol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed that exposure of Xenopus embryos to 0.5 % alcohol from stage 13 to stage 22 produced tadpoles with delayed gut maturation , reduced growth , and down-regulation in several gut developmental genes , with VegT , Pax6 and Sox17 most vulnerable .
	manualset3
200323	5	417337	7	NULL	NULL	0	NULL	stage 13	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed that exposure of Xenopus embryos to 0.5 % alcohol from stage 13 to stage 22 produced tadpoles with delayed gut maturation , reduced growth , and down-regulation in several gut developmental genes , with VegT , Pax6 and Sox17 most vulnerable .
	manualset3
200324	6	417337	7	NULL	NULL	0	NULL	stage 22	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed that exposure of Xenopus embryos to 0.5 % alcohol from stage 13 to stage 22 produced tadpoles with delayed gut maturation , reduced growth , and down-regulation in several gut developmental genes , with VegT , Pax6 and Sox17 most vulnerable .
	manualset3
200325	7	417337	7	NULL	NULL	0	NULL	 tadpoles	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed that exposure of Xenopus embryos to 0.5 % alcohol from stage 13 to stage 22 produced tadpoles with delayed gut maturation , reduced growth , and down-regulation in several gut developmental genes , with VegT , Pax6 and Sox17 most vulnerable .
	manualset3
200326	8	417337	7	NULL	NULL	0	NULL	delayed gut maturation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed that exposure of Xenopus embryos to 0.5 % alcohol from stage 13 to stage 22 produced tadpoles with delayed gut maturation , reduced growth , and down-regulation in several gut developmental genes , with VegT , Pax6 and Sox17 most vulnerable .
	manualset3
200327	9	417337	7	NULL	NULL	0	NULL	reduced growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed that exposure of Xenopus embryos to 0.5 % alcohol from stage 13 to stage 22 produced tadpoles with delayed gut maturation , reduced growth , and down-regulation in several gut developmental genes , with VegT , Pax6 and Sox17 most vulnerable .
	manualset3
200328	10	417337	7	NULL	NULL	0	NULL	down-regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed that exposure of Xenopus embryos to 0.5 % alcohol from stage 13 to stage 22 produced tadpoles with delayed gut maturation , reduced growth , and down-regulation in several gut developmental genes , with VegT , Pax6 and Sox17 most vulnerable .
	manualset3
200329	11	417337	7	NULL	NULL	0	NULL	gut developmental genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed that exposure of Xenopus embryos to 0.5 % alcohol from stage 13 to stage 22 produced tadpoles with delayed gut maturation , reduced growth , and down-regulation in several gut developmental genes , with VegT , Pax6 and Sox17 most vulnerable .
	manualset3
200330	12	417337	7	NULL	NULL	0	NULL	VegT	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed that exposure of Xenopus embryos to 0.5 % alcohol from stage 13 to stage 22 produced tadpoles with delayed gut maturation , reduced growth , and down-regulation in several gut developmental genes , with VegT , Pax6 and Sox17 most vulnerable .
	manualset3
200331	13	417337	7	NULL	NULL	0	NULL	Pax6	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed that exposure of Xenopus embryos to 0.5 % alcohol from stage 13 to stage 22 produced tadpoles with delayed gut maturation , reduced growth , and down-regulation in several gut developmental genes , with VegT , Pax6 and Sox17 most vulnerable .
	manualset3
200332	14	417337	7	NULL	NULL	0	NULL	Sox17	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed that exposure of Xenopus embryos to 0.5 % alcohol from stage 13 to stage 22 produced tadpoles with delayed gut maturation , reduced growth , and down-regulation in several gut developmental genes , with VegT , Pax6 and Sox17 most vulnerable .
	manualset3
200333	1	417338	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed that in such mice FPP was infiltrated with CD8 cells starting from 2 wk posttransplantation and FPP was eventually rejected 8 wk posttransplantation .
	manualset3
200334	2	417338	7	NULL	NULL	0	NULL	FPP	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed that in such mice FPP was infiltrated with CD8 cells starting from 2 wk posttransplantation and FPP was eventually rejected 8 wk posttransplantation .
	manualset3
200335	3	417338	7	NULL	NULL	0	NULL	CD8 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed that in such mice FPP was infiltrated with CD8 cells starting from 2 wk posttransplantation and FPP was eventually rejected 8 wk posttransplantation .
	manualset3
200336	4	417338	7	NULL	NULL	0	NULL	2 wk	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed that in such mice FPP was infiltrated with CD8 cells starting from 2 wk posttransplantation and FPP was eventually rejected 8 wk posttransplantation .
	manualset3
200337	5	417338	7	NULL	NULL	0	NULL	posttransplantation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed that in such mice FPP was infiltrated with CD8 cells starting from 2 wk posttransplantation and FPP was eventually rejected 8 wk posttransplantation .
	manualset3
200338	6	417338	7	NULL	NULL	0	NULL	FPP	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed that in such mice FPP was infiltrated with CD8 cells starting from 2 wk posttransplantation and FPP was eventually rejected 8 wk posttransplantation .
	manualset3
200339	7	417338	7	NULL	NULL	0	NULL	8 wk	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed that in such mice FPP was infiltrated with CD8 cells starting from 2 wk posttransplantation and FPP was eventually rejected 8 wk posttransplantation .
	manualset3
200340	8	417338	7	NULL	NULL	0	NULL	posttransplantation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed that in such mice FPP was infiltrated with CD8 cells starting from 2 wk posttransplantation and FPP was eventually rejected 8 wk posttransplantation .
	manualset3
200343	1	417339	7	NULL	NULL	0	NULL	simple model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We solve analytically a simple model of geometrical positive feedback in which the stress shadow cast by the last large earthquake is progressively fragmented by the increasing tectonic stress .
	manualset3
200344	2	417339	7	NULL	NULL	0	NULL	geometrical positive feedback	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We solve analytically a simple model of geometrical positive feedback in which the stress shadow cast by the last large earthquake is progressively fragmented by the increasing tectonic stress .
	manualset3
200345	3	417339	7	NULL	NULL	0	NULL	stress shadow	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We solve analytically a simple model of geometrical positive feedback in which the stress shadow cast by the last large earthquake is progressively fragmented by the increasing tectonic stress .
	manualset3
200346	4	417339	7	NULL	NULL	0	NULL	last large earthquake	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We solve analytically a simple model of geometrical positive feedback in which the stress shadow cast by the last large earthquake is progressively fragmented by the increasing tectonic stress .
	manualset3
200347	5	417339	7	NULL	NULL	0	NULL	 increasing 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We solve analytically a simple model of geometrical positive feedback in which the stress shadow cast by the last large earthquake is progressively fragmented by the increasing tectonic stress .
	manualset3
200348	6	417339	7	NULL	NULL	0	NULL	tectonic stress	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We solve analytically a simple model of geometrical positive feedback in which the stress shadow cast by the last large earthquake is progressively fragmented by the increasing tectonic stress .
	manualset3
200349	1	417340	7	NULL	NULL	NULL	NULL	 l-ficolin binding reactions	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We sought further insight into l-ficolin binding reactions and MASP-2 activation by passing plasma through GlcNAc-derivatized Sepharose .
	manualset3
200350	2	417340	7	NULL	NULL	0	NULL	MASP-2 activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We sought further insight into l-ficolin binding reactions and MASP-2 activation by passing plasma through GlcNAc-derivatized Sepharose .
	manualset3
200351	3	417340	7	NULL	NULL	0	NULL	plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We sought further insight into l-ficolin binding reactions and MASP-2 activation by passing plasma through GlcNAc-derivatized Sepharose .
	manualset3
200352	4	417340	7	NULL	NULL	NULL	NULL	GlcNAc-derivatized Sepharose	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We sought further insight into l-ficolin binding reactions and MASP-2 activation by passing plasma through GlcNAc-derivatized Sepharose .
	manualset3
200363	1	417341	7	NULL	NULL	0	NULL	endothelial gaps	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	We sought to determine whether endothelial gaps or transcellular holes , similar to those found in leaky vessels in inflammation , could explain the leakiness of tumor vessels .
	manualset3
200364	2	417341	7	NULL	NULL	0	NULL	transcellular holes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	We sought to determine whether endothelial gaps or transcellular holes , similar to those found in leaky vessels in inflammation , could explain the leakiness of tumor vessels .
	manualset3
200365	3	417341	7	NULL	NULL	0	NULL	leaky vessels	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	We sought to determine whether endothelial gaps or transcellular holes , similar to those found in leaky vessels in inflammation , could explain the leakiness of tumor vessels .
	manualset3
200366	4	417341	7	NULL	NULL	0	NULL	inflammation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We sought to determine whether endothelial gaps or transcellular holes , similar to those found in leaky vessels in inflammation , could explain the leakiness of tumor vessels .
	manualset3
200367	5	417341	7	NULL	NULL	0	NULL	 leakiness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We sought to determine whether endothelial gaps or transcellular holes , similar to those found in leaky vessels in inflammation , could explain the leakiness of tumor vessels .
	manualset3
200368	6	417341	7	NULL	NULL	0	NULL	tumor vessels	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We sought to determine whether endothelial gaps or transcellular holes , similar to those found in leaky vessels in inflammation , could explain the leakiness of tumor vessels .
	manualset3
200371	1	417342	7	NULL	NULL	0	NULL	antiinflammatory effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We sought to evaluate the antiinflammatory effects of synthetic human beta-endorphin ( SHB ) when injected into the canine knee joint .
	manualset3
200372	2	417342	7	NULL	NULL	0	NULL	synthetic human beta-endorphin ( SHB )	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	We sought to evaluate the antiinflammatory effects of synthetic human beta-endorphin ( SHB ) when injected into the canine knee joint .
	manualset3
200373	3	417342	7	NULL	NULL	0	NULL	canine knee joint	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We sought to evaluate the antiinflammatory effects of synthetic human beta-endorphin ( SHB ) when injected into the canine knee joint .
	manualset3
200438	1	417343	7	NULL	NULL	0	NULL	engrafting third-party hematopoiesis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	We speculate that the engrafting third-party hematopoiesis produced acute renal allograft rejection with secondary microangiopathic hemolysis through a graft-versus-graft mechanism .
	manualset3
200439	2	417343	7	NULL	NULL	NULL	NULL	acute renal allograft rejection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We speculate that the engrafting third-party hematopoiesis produced acute renal allograft rejection with secondary microangiopathic hemolysis through a graft-versus-graft mechanism .
	manualset3
200440	3	417343	7	NULL	NULL	0	NULL	secondary microangiopathic hemolysis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We speculate that the engrafting third-party hematopoiesis produced acute renal allograft rejection with secondary microangiopathic hemolysis through a graft-versus-graft mechanism .
	manualset3
200441	4	417343	7	NULL	NULL	0	NULL	graft-versus-graft mechanism	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	We speculate that the engrafting third-party hematopoiesis produced acute renal allograft rejection with secondary microangiopathic hemolysis through a graft-versus-graft mechanism .
	manualset3
200442	1	417344	7	NULL	NULL	0	NULL	Tetraodontiformes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We speculated that while Tetraodontiformes evolutionarily lost gastric glands , pufferfish pepsinogen acquired an alternative function to food digestion .
	manualset3
200443	2	417344	7	NULL	NULL	0	NULL	gastric glands	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We speculated that while Tetraodontiformes evolutionarily lost gastric glands , pufferfish pepsinogen acquired an alternative function to food digestion .
	manualset3
200444	3	417344	7	NULL	NULL	0	NULL	pufferfish pepsinogen 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We speculated that while Tetraodontiformes evolutionarily lost gastric glands , pufferfish pepsinogen acquired an alternative function to food digestion .
	manualset3
200445	4	417344	7	NULL	NULL	0	NULL	alternative function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We speculated that while Tetraodontiformes evolutionarily lost gastric glands , pufferfish pepsinogen acquired an alternative function to food digestion .
	manualset3
200446	5	417344	7	NULL	NULL	0	NULL	food digestion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We speculated that while Tetraodontiformes evolutionarily lost gastric glands , pufferfish pepsinogen acquired an alternative function to food digestion .
	manualset3
200447	1	417345	7	NULL	NULL	0	NULL	solid conceptual perspectives	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We strongly recommend using more solid conceptual and theoretical perspectives , as well as more ecologically valid approaches , in designing future studies in emotion expression and perception research .
	manualset3
200448	2	417345	7	NULL	NULL	0	NULL	theoretical perspectives	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We strongly recommend using more solid conceptual and theoretical perspectives , as well as more ecologically valid approaches , in designing future studies in emotion expression and perception research .
	manualset3
200449	3	417345	7	NULL	NULL	0	NULL	ecologically valid approaches	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We strongly recommend using more solid conceptual and theoretical perspectives , as well as more ecologically valid approaches , in designing future studies in emotion expression and perception research .
	manualset3
200450	4	417345	7	NULL	NULL	0	NULL	 future studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We strongly recommend using more solid conceptual and theoretical perspectives , as well as more ecologically valid approaches , in designing future studies in emotion expression and perception research .
	manualset3
200451	5	417345	7	NULL	NULL	0	NULL	emotion expression	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We strongly recommend using more solid conceptual and theoretical perspectives , as well as more ecologically valid approaches , in designing future studies in emotion expression and perception research .
	manualset3
200452	6	417345	7	NULL	NULL	0	NULL	perception research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We strongly recommend using more solid conceptual and theoretical perspectives , as well as more ecologically valid approaches , in designing future studies in emotion expression and perception research .
	manualset3
200453	1	417346	7	NULL	NULL	0	NULL	10 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 10 patients ( mean age 64 ( SE 2 ) years ) with stable moderate to severe chronic heart failure ( ejection fraction 23 ( 3 ) % ) who received PIT , and 10 control patients matched for age and severity .
	manualset3
200454	2	417346	7	NULL	NULL	0	NULL	mean age 64	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 10 patients ( mean age 64 ( SE 2 ) years ) with stable moderate to severe chronic heart failure ( ejection fraction 23 ( 3 ) % ) who received PIT , and 10 control patients matched for age and severity .
	manualset3
200455	3	417346	7	NULL	NULL	0	NULL	( SE 2 ) years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 10 patients ( mean age 64 ( SE 2 ) years ) with stable moderate to severe chronic heart failure ( ejection fraction 23 ( 3 ) % ) who received PIT , and 10 control patients matched for age and severity .
	manualset3
200457	4	417346	7	NULL	NULL	0	NULL	moderate heart failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 10 patients ( mean age 64 ( SE 2 ) years ) with stable moderate to severe chronic heart failure ( ejection fraction 23 ( 3 ) % ) who received PIT , and 10 control patients matched for age and severity .
	manualset3
200458	5	417346	7	NULL	NULL	0	NULL	 severe chronic heart failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 10 patients ( mean age 64 ( SE 2 ) years ) with stable moderate to severe chronic heart failure ( ejection fraction 23 ( 3 ) % ) who received PIT , and 10 control patients matched for age and severity .
	manualset3
200459	6	417346	7	NULL	NULL	0	NULL	 ejection fraction	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 10 patients ( mean age 64 ( SE 2 ) years ) with stable moderate to severe chronic heart failure ( ejection fraction 23 ( 3 ) % ) who received PIT , and 10 control patients matched for age and severity .
	manualset3
200460	7	417346	7	NULL	NULL	0	NULL	23 ( 3 ) %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 10 patients ( mean age 64 ( SE 2 ) years ) with stable moderate to severe chronic heart failure ( ejection fraction 23 ( 3 ) % ) who received PIT , and 10 control patients matched for age and severity .
	manualset3
200461	8	417346	7	NULL	NULL	0	NULL	PIT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 10 patients ( mean age 64 ( SE 2 ) years ) with stable moderate to severe chronic heart failure ( ejection fraction 23 ( 3 ) % ) who received PIT , and 10 control patients matched for age and severity .
	manualset3
200462	9	417346	7	NULL	NULL	0	NULL	10 control patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 10 patients ( mean age 64 ( SE 2 ) years ) with stable moderate to severe chronic heart failure ( ejection fraction 23 ( 3 ) % ) who received PIT , and 10 control patients matched for age and severity .
	manualset3
200463	10	417346	7	NULL	NULL	0	NULL	age	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 10 patients ( mean age 64 ( SE 2 ) years ) with stable moderate to severe chronic heart failure ( ejection fraction 23 ( 3 ) % ) who received PIT , and 10 control patients matched for age and severity .
	manualset3
200464	11	417346	7	NULL	NULL	0	NULL	severity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 10 patients ( mean age 64 ( SE 2 ) years ) with stable moderate to severe chronic heart failure ( ejection fraction 23 ( 3 ) % ) who received PIT , and 10 control patients matched for age and severity .
	manualset3
200465	1	417347	7	NULL	NULL	0	NULL	 12 young subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 12 young subjects ( mean age 10 years ) with steroid-responsive idiopathic nephrotic syndrome and with signs of steroid toxicity .
	manualset3
200466	2	417347	7	NULL	NULL	0	NULL	mean age	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 12 young subjects ( mean age 10 years ) with steroid-responsive idiopathic nephrotic syndrome and with signs of steroid toxicity .
	manualset3
200467	3	417347	7	NULL	NULL	0	NULL	10 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 12 young subjects ( mean age 10 years ) with steroid-responsive idiopathic nephrotic syndrome and with signs of steroid toxicity .
	manualset3
200468	4	417347	7	NULL	NULL	0	NULL	steroid-responsive idiopathic nephrotic syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 12 young subjects ( mean age 10 years ) with steroid-responsive idiopathic nephrotic syndrome and with signs of steroid toxicity .
	manualset3
200469	5	417347	7	NULL	NULL	0	NULL	 signs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 12 young subjects ( mean age 10 years ) with steroid-responsive idiopathic nephrotic syndrome and with signs of steroid toxicity .
	manualset3
200470	6	417347	7	NULL	NULL	0	NULL	steroid toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 12 young subjects ( mean age 10 years ) with steroid-responsive idiopathic nephrotic syndrome and with signs of steroid toxicity .
	manualset3
200471	1	417348	7	NULL	NULL	0	NULL	18 adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 18 adults with FMRI while they performed grammatical transformations of varying complexity levels ( 2-letter , 3-letter , and 4-letter sentences ) .
	manualset3
200472	2	417348	7	NULL	NULL	0	NULL	FMRI 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 18 adults with FMRI while they performed grammatical transformations of varying complexity levels ( 2-letter , 3-letter , and 4-letter sentences ) .
	manualset3
200473	3	417348	7	NULL	NULL	0	NULL	grammatical transformations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 18 adults with FMRI while they performed grammatical transformations of varying complexity levels ( 2-letter , 3-letter , and 4-letter sentences ) .
	manualset3
200474	4	417348	7	NULL	NULL	0	NULL	complexity levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 18 adults with FMRI while they performed grammatical transformations of varying complexity levels ( 2-letter , 3-letter , and 4-letter sentences ) .
	manualset3
200475	5	417348	7	NULL	NULL	0	NULL	2-letter sentences	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 18 adults with FMRI while they performed grammatical transformations of varying complexity levels ( 2-letter , 3-letter , and 4-letter sentences ) .
	manualset3
200476	6	417348	7	NULL	NULL	0	NULL	3-letter sentences	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 18 adults with FMRI while they performed grammatical transformations of varying complexity levels ( 2-letter , 3-letter , and 4-letter sentences ) .
	manualset3
200477	7	417348	7	NULL	NULL	0	NULL	4-letter sentences	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 18 adults with FMRI while they performed grammatical transformations of varying complexity levels ( 2-letter , 3-letter , and 4-letter sentences ) .
	manualset3
200478	1	417349	7	NULL	NULL	0	NULL	318 consecutive patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 318 consecutive patients suffering from stroke .
	manualset3
200479	2	417349	7	NULL	NULL	0	NULL	stroke	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 318 consecutive patients suffering from stroke .
	manualset3
200480	1	417350	7	NULL	NULL	0	NULL	RBCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied RBCs from healthy volunteers ( n = 10 ) and from patients with ( n = 15 ) and without ( n = 9 ) sepsis within 24 h of intensive care unit admission and also on day 3 for the septic patients .
	manualset3
200481	2	417350	7	NULL	NULL	0	NULL	healthy volunteers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied RBCs from healthy volunteers ( n = 10 ) and from patients with ( n = 15 ) and without ( n = 9 ) sepsis within 24 h of intensive care unit admission and also on day 3 for the septic patients .
	manualset3
200482	3	417350	7	NULL	NULL	0	NULL	n = 10	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied RBCs from healthy volunteers ( n = 10 ) and from patients with ( n = 15 ) and without ( n = 9 ) sepsis within 24 h of intensive care unit admission and also on day 3 for the septic patients .
	manualset3
200483	4	417350	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied RBCs from healthy volunteers ( n = 10 ) and from patients with ( n = 15 ) and without ( n = 9 ) sepsis within 24 h of intensive care unit admission and also on day 3 for the septic patients .
	manualset3
200484	5	417350	7	NULL	NULL	0	NULL	n = 15	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied RBCs from healthy volunteers ( n = 10 ) and from patients with ( n = 15 ) and without ( n = 9 ) sepsis within 24 h of intensive care unit admission and also on day 3 for the septic patients .
	manualset3
200485	6	417350	7	NULL	NULL	0	NULL	n = 9	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied RBCs from healthy volunteers ( n = 10 ) and from patients with ( n = 15 ) and without ( n = 9 ) sepsis within 24 h of intensive care unit admission and also on day 3 for the septic patients .
	manualset3
200486	7	417350	7	NULL	NULL	0	NULL	sepsis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied RBCs from healthy volunteers ( n = 10 ) and from patients with ( n = 15 ) and without ( n = 9 ) sepsis within 24 h of intensive care unit admission and also on day 3 for the septic patients .
	manualset3
200487	8	417350	7	NULL	NULL	0	NULL	24h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied RBCs from healthy volunteers ( n = 10 ) and from patients with ( n = 15 ) and without ( n = 9 ) sepsis within 24 h of intensive care unit admission and also on day 3 for the septic patients .
	manualset3
200488	9	417350	7	NULL	NULL	0	NULL	intensive care unit admission	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied RBCs from healthy volunteers ( n = 10 ) and from patients with ( n = 15 ) and without ( n = 9 ) sepsis within 24 h of intensive care unit admission and also on day 3 for the septic patients .
	manualset3
200489	10	417350	7	NULL	NULL	0	NULL	day 3	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied RBCs from healthy volunteers ( n = 10 ) and from patients with ( n = 15 ) and without ( n = 9 ) sepsis within 24 h of intensive care unit admission and also on day 3 for the septic patients .
	manualset3
200490	11	417350	7	NULL	NULL	0	NULL	septic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied RBCs from healthy volunteers ( n = 10 ) and from patients with ( n = 15 ) and without ( n = 9 ) sepsis within 24 h of intensive care unit admission and also on day 3 for the septic patients .
	manualset3
200491	1	417351	7	NULL	NULL	0	NULL	large Danish family	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied a large Danish family of seven generations in which autosomal dominant retinitis pigmentosa ( adRP ) , a heterogeneous genetic form of retinal dystrophy , was segregating .
	manualset3
200492	2	417351	7	NULL	NULL	0	NULL	seven generations	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied a large Danish family of seven generations in which autosomal dominant retinitis pigmentosa ( adRP ) , a heterogeneous genetic form of retinal dystrophy , was segregating .
	manualset3
200493	3	417351	7	NULL	NULL	0	NULL	 autosomal dominant retinitis pigmentosa ( adRP )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied a large Danish family of seven generations in which autosomal dominant retinitis pigmentosa ( adRP ) , a heterogeneous genetic form of retinal dystrophy , was segregating .
	manualset3
200494	4	417351	7	NULL	NULL	0	NULL	heterogeneous genetic form	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied a large Danish family of seven generations in which autosomal dominant retinitis pigmentosa ( adRP ) , a heterogeneous genetic form of retinal dystrophy , was segregating .
	manualset3
200495	5	417351	7	NULL	NULL	0	NULL	retinal dystrophy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied a large Danish family of seven generations in which autosomal dominant retinitis pigmentosa ( adRP ) , a heterogeneous genetic form of retinal dystrophy , was segregating .
	manualset3
200496	1	417352	7	NULL	NULL	0	NULL	T1N0M0 breast cancers	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied all the T1N0M0 breast cancers that had led to recurrency or death ( n = 21 , 95 % T1cN0M0 ) during the follow-up period ( 4-14 years ) .
	manualset3
200497	2	417352	7	NULL	NULL	0	NULL	 death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied all the T1N0M0 breast cancers that had led to recurrency or death ( n = 21 , 95 % T1cN0M0 ) during the follow-up period ( 4-14 years ) .
	manualset3
200498	3	417352	7	NULL	NULL	0	NULL	n = 21	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied all the T1N0M0 breast cancers that had led to recurrency or death ( n = 21 , 95 % T1cN0M0 ) during the follow-up period ( 4-14 years ) .
	manualset3
200499	4	417352	7	NULL	NULL	0	NULL	95 % T1cN0M0	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied all the T1N0M0 breast cancers that had led to recurrency or death ( n = 21 , 95 % T1cN0M0 ) during the follow-up period ( 4-14 years ) .
	manualset3
200500	5	417352	7	NULL	NULL	0	NULL	follow-up period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied all the T1N0M0 breast cancers that had led to recurrency or death ( n = 21 , 95 % T1cN0M0 ) during the follow-up period ( 4-14 years ) .
	manualset3
200501	6	417352	7	NULL	NULL	0	NULL	 4-14 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied all the T1N0M0 breast cancers that had led to recurrency or death ( n = 21 , 95 % T1cN0M0 ) during the follow-up period ( 4-14 years ) .
	manualset3
200502	1	417353	7	NULL	NULL	0	NULL	brain areas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied coherence between brain areas known to be linked by two different types of connections : ( i ) dense narrow bands of long corticocortical fibers ; ( ii ) broad complex networks of corticocortical and corticosubcortical fibers .
	manualset3
200503	2	417353	7	NULL	NULL	NULL	NULL	two different types of connections	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We studied coherence between brain areas known to be linked by two different types of connections : ( i ) dense narrow bands of long corticocortical fibers ; ( ii ) broad complex networks of corticocortical and corticosubcortical fibers .
	manualset3
200505	4	417353	7	NULL	NULL	NULL	NULL	dense narrow bands	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We studied coherence between brain areas known to be linked by two different types of connections : ( i ) dense narrow bands of long corticocortical fibers ; ( ii ) broad complex networks of corticocortical and corticosubcortical fibers .
	manualset3
200506	5	417353	7	NULL	NULL	0	NULL	long corticocortical fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied coherence between brain areas known to be linked by two different types of connections : ( i ) dense narrow bands of long corticocortical fibers ; ( ii ) broad complex networks of corticocortical and corticosubcortical fibers .
	manualset3
200507	6	417353	7	NULL	NULL	0	NULL	broad complex networks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied coherence between brain areas known to be linked by two different types of connections : ( i ) dense narrow bands of long corticocortical fibers ; ( ii ) broad complex networks of corticocortical and corticosubcortical fibers .
	manualset3
200508	7	417353	7	NULL	NULL	0	NULL	corticocortical fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied coherence between brain areas known to be linked by two different types of connections : ( i ) dense narrow bands of long corticocortical fibers ; ( ii ) broad complex networks of corticocortical and corticosubcortical fibers .
	manualset3
200509	8	417353	7	NULL	NULL	0	NULL	corticosubcortical fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied coherence between brain areas known to be linked by two different types of connections : ( i ) dense narrow bands of long corticocortical fibers ; ( ii ) broad complex networks of corticocortical and corticosubcortical fibers .
	manualset3
203014	9	417353	7	NULL	NULL	0	NULL	coherence	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied coherence between brain areas known to be linked by two different types of connections : ( i ) dense narrow bands of long corticocortical fibers ; ( ii ) broad complex networks of corticocortical and corticosubcortical fibers .
	manualset3
200519	1	417354	7	NULL	NULL	0	NULL	dental caries susceptibility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied dental caries susceptibility in various inbred mice strains infected with Streptococcus mutans and the inheritance pattern in the F1 and the N2 backcross animals .
	manualset3
200520	2	417354	7	NULL	NULL	0	NULL	 inbred mice strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied dental caries susceptibility in various inbred mice strains infected with Streptococcus mutans and the inheritance pattern in the F1 and the N2 backcross animals .
	manualset3
200521	3	417354	7	NULL	NULL	0	NULL	Streptococcus mutans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied dental caries susceptibility in various inbred mice strains infected with Streptococcus mutans and the inheritance pattern in the F1 and the N2 backcross animals .
	manualset3
200522	4	417354	7	NULL	NULL	0	NULL	inheritance pattern	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied dental caries susceptibility in various inbred mice strains infected with Streptococcus mutans and the inheritance pattern in the F1 and the N2 backcross animals .
	manualset3
200523	5	417354	7	NULL	NULL	0	NULL	F1 backcross animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied dental caries susceptibility in various inbred mice strains infected with Streptococcus mutans and the inheritance pattern in the F1 and the N2 backcross animals .
	manualset3
200524	6	417354	7	NULL	NULL	0	NULL	N2 backcross animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied dental caries susceptibility in various inbred mice strains infected with Streptococcus mutans and the inheritance pattern in the F1 and the N2 backcross animals .
	manualset3
200525	1	417355	7	NULL	NULL	NULL	NULL	 in vitro cytokine production	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We studied in vitro cytokine production by peripheral blood mononuclear cells ( PBMC ) from patients with primary and recurrent hydatid disease when cells were incubated with mitogen ( PHA ) and antigen from hydatid cyst fluid ( HCFAg ) ; levels of specific IgE , IgG4 and eosinophil counts were also measured in sera .
	manualset3
200527	2	417355	7	NULL	NULL	0	NULL	peripheral blood mononuclear cells ( PBMC )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in vitro cytokine production by peripheral blood mononuclear cells ( PBMC ) from patients with primary and recurrent hydatid disease when cells were incubated with mitogen ( PHA ) and antigen from hydatid cyst fluid ( HCFAg ) ; levels of specific IgE , IgG4 and eosinophil counts were also measured in sera .
	manualset3
200529	3	417355	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in vitro cytokine production by peripheral blood mononuclear cells ( PBMC ) from patients with primary and recurrent hydatid disease when cells were incubated with mitogen ( PHA ) and antigen from hydatid cyst fluid ( HCFAg ) ; levels of specific IgE , IgG4 and eosinophil counts were also measured in sera .
	manualset3
200531	4	417355	7	NULL	NULL	0	NULL	primary hydatid disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in vitro cytokine production by peripheral blood mononuclear cells ( PBMC ) from patients with primary and recurrent hydatid disease when cells were incubated with mitogen ( PHA ) and antigen from hydatid cyst fluid ( HCFAg ) ; levels of specific IgE , IgG4 and eosinophil counts were also measured in sera .
	manualset3
200532	5	417355	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in vitro cytokine production by peripheral blood mononuclear cells ( PBMC ) from patients with primary and recurrent hydatid disease when cells were incubated with mitogen ( PHA ) and antigen from hydatid cyst fluid ( HCFAg ) ; levels of specific IgE , IgG4 and eosinophil counts were also measured in sera .
	manualset3
200534	6	417355	7	NULL	NULL	NULL	NULL	mitogen	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We studied in vitro cytokine production by peripheral blood mononuclear cells ( PBMC ) from patients with primary and recurrent hydatid disease when cells were incubated with mitogen ( PHA ) and antigen from hydatid cyst fluid ( HCFAg ) ; levels of specific IgE , IgG4 and eosinophil counts were also measured in sera .
	manualset3
200538	7	417355	7	NULL	NULL	0	NULL	PHA 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in vitro cytokine production by peripheral blood mononuclear cells ( PBMC ) from patients with primary and recurrent hydatid disease when cells were incubated with mitogen ( PHA ) and antigen from hydatid cyst fluid ( HCFAg ) ; levels of specific IgE , IgG4 and eosinophil counts were also measured in sera .
	manualset3
200540	8	417355	7	NULL	NULL	0	NULL	antigen	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in vitro cytokine production by peripheral blood mononuclear cells ( PBMC ) from patients with primary and recurrent hydatid disease when cells were incubated with mitogen ( PHA ) and antigen from hydatid cyst fluid ( HCFAg ) ; levels of specific IgE , IgG4 and eosinophil counts were also measured in sera .
	manualset3
200541	9	417355	7	NULL	NULL	0	NULL	hydatid cyst fluid ( HCFAg ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in vitro cytokine production by peripheral blood mononuclear cells ( PBMC ) from patients with primary and recurrent hydatid disease when cells were incubated with mitogen ( PHA ) and antigen from hydatid cyst fluid ( HCFAg ) ; levels of specific IgE , IgG4 and eosinophil counts were also measured in sera .
	manualset3
200542	10	417355	7	NULL	NULL	0	NULL	 levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in vitro cytokine production by peripheral blood mononuclear cells ( PBMC ) from patients with primary and recurrent hydatid disease when cells were incubated with mitogen ( PHA ) and antigen from hydatid cyst fluid ( HCFAg ) ; levels of specific IgE , IgG4 and eosinophil counts were also measured in sera .
	manualset3
200543	11	417355	7	NULL	NULL	0	NULL	IgE counts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in vitro cytokine production by peripheral blood mononuclear cells ( PBMC ) from patients with primary and recurrent hydatid disease when cells were incubated with mitogen ( PHA ) and antigen from hydatid cyst fluid ( HCFAg ) ; levels of specific IgE , IgG4 and eosinophil counts were also measured in sera .
	manualset3
200544	12	417355	7	NULL	NULL	0	NULL	IgG4 counts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in vitro cytokine production by peripheral blood mononuclear cells ( PBMC ) from patients with primary and recurrent hydatid disease when cells were incubated with mitogen ( PHA ) and antigen from hydatid cyst fluid ( HCFAg ) ; levels of specific IgE , IgG4 and eosinophil counts were also measured in sera .
	manualset3
200545	13	417355	7	NULL	NULL	0	NULL	eosinophil counts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in vitro cytokine production by peripheral blood mononuclear cells ( PBMC ) from patients with primary and recurrent hydatid disease when cells were incubated with mitogen ( PHA ) and antigen from hydatid cyst fluid ( HCFAg ) ; levels of specific IgE , IgG4 and eosinophil counts were also measured in sera .
	manualset3
200546	14	417355	7	NULL	NULL	0	NULL	sera	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in vitro cytokine production by peripheral blood mononuclear cells ( PBMC ) from patients with primary and recurrent hydatid disease when cells were incubated with mitogen ( PHA ) and antigen from hydatid cyst fluid ( HCFAg ) ; levels of specific IgE , IgG4 and eosinophil counts were also measured in sera .
	manualset3
200547	15	417355	7	NULL	NULL	0	NULL	 recurrent hydatid disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in vitro cytokine production by peripheral blood mononuclear cells ( PBMC ) from patients with primary and recurrent hydatid disease when cells were incubated with mitogen ( PHA ) and antigen from hydatid cyst fluid ( HCFAg ) ; levels of specific IgE , IgG4 and eosinophil counts were also measured in sera .
	manualset3
200548	1	417356	7	NULL	NULL	0	NULL	parameters 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied parameters of cellular immunity in 23 schizophrenic patients and compared them to 16 matched healthy controls and to 12 patients with rheumatoid arthritis ( RA ) .
	manualset3
200549	2	417356	7	NULL	NULL	0	NULL	cellular immunity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied parameters of cellular immunity in 23 schizophrenic patients and compared them to 16 matched healthy controls and to 12 patients with rheumatoid arthritis ( RA ) .
	manualset3
200550	3	417356	7	NULL	NULL	0	NULL	23 schizophrenic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied parameters of cellular immunity in 23 schizophrenic patients and compared them to 16 matched healthy controls and to 12 patients with rheumatoid arthritis ( RA ) .
	manualset3
200551	4	417356	7	NULL	NULL	0	NULL	16 matched healthy controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied parameters of cellular immunity in 23 schizophrenic patients and compared them to 16 matched healthy controls and to 12 patients with rheumatoid arthritis ( RA ) .
	manualset3
200552	5	417356	7	NULL	NULL	0	NULL	12 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied parameters of cellular immunity in 23 schizophrenic patients and compared them to 16 matched healthy controls and to 12 patients with rheumatoid arthritis ( RA ) .
	manualset3
200553	6	417356	7	NULL	NULL	0	NULL	rheumatoid arthritis ( RA )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied parameters of cellular immunity in 23 schizophrenic patients and compared them to 16 matched healthy controls and to 12 patients with rheumatoid arthritis ( RA ) .
	manualset3
200556	1	417357	7	NULL	NULL	0	NULL	changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the changes in plasma cytokine ( IL-6 and IL-8 ) levels during lung surgery in 20 patients .
	manualset3
200558	2	417357	7	NULL	NULL	0	NULL	plasma cytokine levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the changes in plasma cytokine ( IL-6 and IL-8 ) levels during lung surgery in 20 patients .
	manualset3
200560	3	417357	7	NULL	NULL	0	NULL	 IL-6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the changes in plasma cytokine ( IL-6 and IL-8 ) levels during lung surgery in 20 patients .
	manualset3
200562	4	417357	7	NULL	NULL	0	NULL	 IL-8	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the changes in plasma cytokine ( IL-6 and IL-8 ) levels during lung surgery in 20 patients .
	manualset3
200563	5	417357	7	NULL	NULL	0	NULL	lung surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the changes in plasma cytokine ( IL-6 and IL-8 ) levels during lung surgery in 20 patients .
	manualset3
200566	6	417357	7	NULL	NULL	0	NULL	 20 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the changes in plasma cytokine ( IL-6 and IL-8 ) levels during lung surgery in 20 patients .
	manualset3
200571	1	417358	7	NULL	NULL	0	NULL	contractile response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the contractile response of isolated rat left ventricular papillary muscles to isoproterenol and the effect of angiotensin II on this response .
	manualset3
200579	2	417358	7	NULL	NULL	0	NULL	 isolated rat left ventricular papillary muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the contractile response of isolated rat left ventricular papillary muscles to isoproterenol and the effect of angiotensin II on this response .
	manualset3
200580	3	417358	7	NULL	NULL	0	NULL	 isoproterenol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the contractile response of isolated rat left ventricular papillary muscles to isoproterenol and the effect of angiotensin II on this response .
	manualset3
200582	4	417358	7	NULL	NULL	0	NULL	effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the contractile response of isolated rat left ventricular papillary muscles to isoproterenol and the effect of angiotensin II on this response .
	manualset3
200583	5	417358	7	NULL	NULL	0	NULL	angiotensin II 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the contractile response of isolated rat left ventricular papillary muscles to isoproterenol and the effect of angiotensin II on this response .
	manualset3
200584	6	417358	7	NULL	NULL	0	NULL	 response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the contractile response of isolated rat left ventricular papillary muscles to isoproterenol and the effect of angiotensin II on this response .
	manualset3
200590	1	417359	7	NULL	NULL	0	NULL	effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the effects of dl-alpha-difluoromethylarginine ( DFMA ) and dl-alpha-difluoromethylornithine ( DFMO ) , specific , irreversible inhibitors of arginine decarboxylase ( ADC ) and ornithine decarboxylase ( ODC ) , respectively , on organogenesis growth and titers of free polyamines and conjugated putrescines ( hydroxycinnamoyl putrescines ) in tobacco ( Nicotiana tabacum cv Xanthi n.c. ) calli .
	manualset3
200592	2	417359	7	NULL	NULL	0	NULL	dl-alpha-difluoromethylarginine ( DFMA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the effects of dl-alpha-difluoromethylarginine ( DFMA ) and dl-alpha-difluoromethylornithine ( DFMO ) , specific , irreversible inhibitors of arginine decarboxylase ( ADC ) and ornithine decarboxylase ( ODC ) , respectively , on organogenesis growth and titers of free polyamines and conjugated putrescines ( hydroxycinnamoyl putrescines ) in tobacco ( Nicotiana tabacum cv Xanthi n.c. ) calli .
	manualset3
200594	3	417359	7	NULL	NULL	0	NULL	dl-alpha-difluoromethylornithine ( DFMO )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the effects of dl-alpha-difluoromethylarginine ( DFMA ) and dl-alpha-difluoromethylornithine ( DFMO ) , specific , irreversible inhibitors of arginine decarboxylase ( ADC ) and ornithine decarboxylase ( ODC ) , respectively , on organogenesis growth and titers of free polyamines and conjugated putrescines ( hydroxycinnamoyl putrescines ) in tobacco ( Nicotiana tabacum cv Xanthi n.c. ) calli .
	manualset3
200595	4	417359	7	NULL	NULL	0	NULL	irreversible inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the effects of dl-alpha-difluoromethylarginine ( DFMA ) and dl-alpha-difluoromethylornithine ( DFMO ) , specific , irreversible inhibitors of arginine decarboxylase ( ADC ) and ornithine decarboxylase ( ODC ) , respectively , on organogenesis growth and titers of free polyamines and conjugated putrescines ( hydroxycinnamoyl putrescines ) in tobacco ( Nicotiana tabacum cv Xanthi n.c. ) calli .
	manualset3
200596	5	417359	7	NULL	NULL	0	NULL	arginine decarboxylase ( ADC )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the effects of dl-alpha-difluoromethylarginine ( DFMA ) and dl-alpha-difluoromethylornithine ( DFMO ) , specific , irreversible inhibitors of arginine decarboxylase ( ADC ) and ornithine decarboxylase ( ODC ) , respectively , on organogenesis growth and titers of free polyamines and conjugated putrescines ( hydroxycinnamoyl putrescines ) in tobacco ( Nicotiana tabacum cv Xanthi n.c. ) calli .
	manualset3
200599	6	417359	7	NULL	NULL	0	NULL	ornithine decarboxylase ( ODC )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the effects of dl-alpha-difluoromethylarginine ( DFMA ) and dl-alpha-difluoromethylornithine ( DFMO ) , specific , irreversible inhibitors of arginine decarboxylase ( ADC ) and ornithine decarboxylase ( ODC ) , respectively , on organogenesis growth and titers of free polyamines and conjugated putrescines ( hydroxycinnamoyl putrescines ) in tobacco ( Nicotiana tabacum cv Xanthi n.c. ) calli .
	manualset3
200601	7	417359	7	NULL	NULL	0	NULL	organogenesis growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the effects of dl-alpha-difluoromethylarginine ( DFMA ) and dl-alpha-difluoromethylornithine ( DFMO ) , specific , irreversible inhibitors of arginine decarboxylase ( ADC ) and ornithine decarboxylase ( ODC ) , respectively , on organogenesis growth and titers of free polyamines and conjugated putrescines ( hydroxycinnamoyl putrescines ) in tobacco ( Nicotiana tabacum cv Xanthi n.c. ) calli .
	manualset3
200602	8	417359	7	NULL	NULL	0	NULL	titers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the effects of dl-alpha-difluoromethylarginine ( DFMA ) and dl-alpha-difluoromethylornithine ( DFMO ) , specific , irreversible inhibitors of arginine decarboxylase ( ADC ) and ornithine decarboxylase ( ODC ) , respectively , on organogenesis growth and titers of free polyamines and conjugated putrescines ( hydroxycinnamoyl putrescines ) in tobacco ( Nicotiana tabacum cv Xanthi n.c. ) calli .
	manualset3
200603	9	417359	7	NULL	NULL	0	NULL	free polyamines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the effects of dl-alpha-difluoromethylarginine ( DFMA ) and dl-alpha-difluoromethylornithine ( DFMO ) , specific , irreversible inhibitors of arginine decarboxylase ( ADC ) and ornithine decarboxylase ( ODC ) , respectively , on organogenesis growth and titers of free polyamines and conjugated putrescines ( hydroxycinnamoyl putrescines ) in tobacco ( Nicotiana tabacum cv Xanthi n.c. ) calli .
	manualset3
200604	10	417359	7	NULL	NULL	0	NULL	conjugated putrescines ( hydroxycinnamoyl putrescines )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the effects of dl-alpha-difluoromethylarginine ( DFMA ) and dl-alpha-difluoromethylornithine ( DFMO ) , specific , irreversible inhibitors of arginine decarboxylase ( ADC ) and ornithine decarboxylase ( ODC ) , respectively , on organogenesis growth and titers of free polyamines and conjugated putrescines ( hydroxycinnamoyl putrescines ) in tobacco ( Nicotiana tabacum cv Xanthi n.c. ) calli .
	manualset3
200605	11	417359	7	NULL	NULL	0	NULL	tobacco	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the effects of dl-alpha-difluoromethylarginine ( DFMA ) and dl-alpha-difluoromethylornithine ( DFMO ) , specific , irreversible inhibitors of arginine decarboxylase ( ADC ) and ornithine decarboxylase ( ODC ) , respectively , on organogenesis growth and titers of free polyamines and conjugated putrescines ( hydroxycinnamoyl putrescines ) in tobacco ( Nicotiana tabacum cv Xanthi n.c. ) calli .
	manualset3
200606	12	417359	7	NULL	NULL	0	NULL	Nicotiana tabacum cv Xanthi n.c. ) calli 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the effects of dl-alpha-difluoromethylarginine ( DFMA ) and dl-alpha-difluoromethylornithine ( DFMO ) , specific , irreversible inhibitors of arginine decarboxylase ( ADC ) and ornithine decarboxylase ( ODC ) , respectively , on organogenesis growth and titers of free polyamines and conjugated putrescines ( hydroxycinnamoyl putrescines ) in tobacco ( Nicotiana tabacum cv Xanthi n.c. ) calli .
	manualset3
200607	1	417360	7	NULL	NULL	0	NULL	galactosylated proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All galactosylated proteins were dose-dependently taken up by the liver and the relative amount accumulated in the liver was decreased with an increase of the administered dose .
	manualset3
200608	2	417360	7	NULL	NULL	0	NULL	 liver 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	All galactosylated proteins were dose-dependently taken up by the liver and the relative amount accumulated in the liver was decreased with an increase of the administered dose .
	manualset3
200609	3	417360	7	NULL	NULL	0	NULL	relative amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All galactosylated proteins were dose-dependently taken up by the liver and the relative amount accumulated in the liver was decreased with an increase of the administered dose .
	manualset3
200610	4	417360	7	NULL	NULL	0	NULL	 liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	All galactosylated proteins were dose-dependently taken up by the liver and the relative amount accumulated in the liver was decreased with an increase of the administered dose .
	manualset3
200611	5	417360	7	NULL	NULL	0	NULL	 increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All galactosylated proteins were dose-dependently taken up by the liver and the relative amount accumulated in the liver was decreased with an increase of the administered dose .
	manualset3
200612	6	417360	7	NULL	NULL	0	NULL	administered dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All galactosylated proteins were dose-dependently taken up by the liver and the relative amount accumulated in the liver was decreased with an increase of the administered dose .
	manualset3
200613	1	417361	7	NULL	NULL	0	NULL	 effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the effects of insulin and insulin-like growth factor-1 ( IGF-1 ) on the growth of porcine vascular smooth muscle cells and on the synthesis of extracellular matrix .
	manualset3
200614	2	417361	7	NULL	NULL	0	NULL	insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the effects of insulin and insulin-like growth factor-1 ( IGF-1 ) on the growth of porcine vascular smooth muscle cells and on the synthesis of extracellular matrix .
	manualset3
200615	3	417361	7	NULL	NULL	0	NULL	insulin-like growth factor-1 ( IGF-1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the effects of insulin and insulin-like growth factor-1 ( IGF-1 ) on the growth of porcine vascular smooth muscle cells and on the synthesis of extracellular matrix .
	manualset3
200616	4	417361	7	NULL	NULL	0	NULL	growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the effects of insulin and insulin-like growth factor-1 ( IGF-1 ) on the growth of porcine vascular smooth muscle cells and on the synthesis of extracellular matrix .
	manualset3
200617	5	417361	7	NULL	NULL	0	NULL	porcine vascular smooth muscle cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the effects of insulin and insulin-like growth factor-1 ( IGF-1 ) on the growth of porcine vascular smooth muscle cells and on the synthesis of extracellular matrix .
	manualset3
200618	6	417361	7	NULL	NULL	0	NULL	 synthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the effects of insulin and insulin-like growth factor-1 ( IGF-1 ) on the growth of porcine vascular smooth muscle cells and on the synthesis of extracellular matrix .
	manualset3
200619	7	417361	7	NULL	NULL	0	NULL	extracellular matrix 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the effects of insulin and insulin-like growth factor-1 ( IGF-1 ) on the growth of porcine vascular smooth muscle cells and on the synthesis of extracellular matrix .
	manualset3
200620	1	417362	7	NULL	NULL	NULL	NULL	effects	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We studied the effects of milrinone and its mechanism in nonfatigued and fatigued diaphragms in dogs .
	manualset3
200621	2	417362	7	NULL	NULL	0	NULL	milrinone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the effects of milrinone and its mechanism in nonfatigued and fatigued diaphragms in dogs .
	manualset3
200622	3	417362	7	NULL	NULL	0	NULL	mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the effects of milrinone and its mechanism in nonfatigued and fatigued diaphragms in dogs .
	manualset3
200623	4	417362	7	NULL	NULL	0	NULL	nonfatigued  diaphragms	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the effects of milrinone and its mechanism in nonfatigued and fatigued diaphragms in dogs .
	manualset3
200624	5	417362	7	NULL	NULL	0	NULL	 fatigued diaphragms	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the effects of milrinone and its mechanism in nonfatigued and fatigued diaphragms in dogs .
	manualset3
200625	6	417362	7	NULL	NULL	0	NULL	dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the effects of milrinone and its mechanism in nonfatigued and fatigued diaphragms in dogs .
	manualset3
200626	1	417363	7	NULL	NULL	0	NULL	mucosa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the mucosa close to the carcinoma of large bowel ( CLB ) in 200 cases , the carcinoma tissue of CLB in 130 and the mucosa of fetus large bowel in 24 by mucin histochemistry , in addition to the mucosa near CLB studied by scanning electron microscope ( SEM ) in 25 .
	manualset3
200627	2	417363	7	NULL	NULL	0	NULL	carcinoma of large bowel ( CLB )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the mucosa close to the carcinoma of large bowel ( CLB ) in 200 cases , the carcinoma tissue of CLB in 130 and the mucosa of fetus large bowel in 24 by mucin histochemistry , in addition to the mucosa near CLB studied by scanning electron microscope ( SEM ) in 25 .
	manualset3
200628	3	417363	7	NULL	NULL	0	NULL	200 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the mucosa close to the carcinoma of large bowel ( CLB ) in 200 cases , the carcinoma tissue of CLB in 130 and the mucosa of fetus large bowel in 24 by mucin histochemistry , in addition to the mucosa near CLB studied by scanning electron microscope ( SEM ) in 25 .
	manualset3
200629	4	417363	7	NULL	NULL	0	NULL	carcinoma tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the mucosa close to the carcinoma of large bowel ( CLB ) in 200 cases , the carcinoma tissue of CLB in 130 and the mucosa of fetus large bowel in 24 by mucin histochemistry , in addition to the mucosa near CLB studied by scanning electron microscope ( SEM ) in 25 .
	manualset3
200630	5	417363	7	NULL	NULL	0	NULL	CLB	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the mucosa close to the carcinoma of large bowel ( CLB ) in 200 cases , the carcinoma tissue of CLB in 130 and the mucosa of fetus large bowel in 24 by mucin histochemistry , in addition to the mucosa near CLB studied by scanning electron microscope ( SEM ) in 25 .
	manualset3
200631	6	417363	7	NULL	NULL	NULL	NULL	130	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We studied the mucosa close to the carcinoma of large bowel ( CLB ) in 200 cases , the carcinoma tissue of CLB in 130 and the mucosa of fetus large bowel in 24 by mucin histochemistry , in addition to the mucosa near CLB studied by scanning electron microscope ( SEM ) in 25 .
	manualset3
200632	7	417363	7	NULL	NULL	0	NULL	mucosa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the mucosa close to the carcinoma of large bowel ( CLB ) in 200 cases , the carcinoma tissue of CLB in 130 and the mucosa of fetus large bowel in 24 by mucin histochemistry , in addition to the mucosa near CLB studied by scanning electron microscope ( SEM ) in 25 .
	manualset3
200633	8	417363	7	NULL	NULL	0	NULL	 fetus large bowel	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the mucosa close to the carcinoma of large bowel ( CLB ) in 200 cases , the carcinoma tissue of CLB in 130 and the mucosa of fetus large bowel in 24 by mucin histochemistry , in addition to the mucosa near CLB studied by scanning electron microscope ( SEM ) in 25 .
	manualset3
200634	9	417363	7	NULL	NULL	0	NULL	24	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the mucosa close to the carcinoma of large bowel ( CLB ) in 200 cases , the carcinoma tissue of CLB in 130 and the mucosa of fetus large bowel in 24 by mucin histochemistry , in addition to the mucosa near CLB studied by scanning electron microscope ( SEM ) in 25 .
	manualset3
200635	10	417363	7	NULL	NULL	0	NULL	mucin histochemistry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the mucosa close to the carcinoma of large bowel ( CLB ) in 200 cases , the carcinoma tissue of CLB in 130 and the mucosa of fetus large bowel in 24 by mucin histochemistry , in addition to the mucosa near CLB studied by scanning electron microscope ( SEM ) in 25 .
	manualset3
200636	11	417363	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the mucosa close to the carcinoma of large bowel ( CLB ) in 200 cases , the carcinoma tissue of CLB in 130 and the mucosa of fetus large bowel in 24 by mucin histochemistry , in addition to the mucosa near CLB studied by scanning electron microscope ( SEM ) in 25 .
	manualset3
200637	12	417363	7	NULL	NULL	0	NULL	mucosa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the mucosa close to the carcinoma of large bowel ( CLB ) in 200 cases , the carcinoma tissue of CLB in 130 and the mucosa of fetus large bowel in 24 by mucin histochemistry , in addition to the mucosa near CLB studied by scanning electron microscope ( SEM ) in 25 .
	manualset3
200638	13	417363	7	NULL	NULL	0	NULL	CLB	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the mucosa close to the carcinoma of large bowel ( CLB ) in 200 cases , the carcinoma tissue of CLB in 130 and the mucosa of fetus large bowel in 24 by mucin histochemistry , in addition to the mucosa near CLB studied by scanning electron microscope ( SEM ) in 25 .
	manualset3
200639	14	417363	7	NULL	NULL	0	NULL	scanning electron microscope ( SEM ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the mucosa close to the carcinoma of large bowel ( CLB ) in 200 cases , the carcinoma tissue of CLB in 130 and the mucosa of fetus large bowel in 24 by mucin histochemistry , in addition to the mucosa near CLB studied by scanning electron microscope ( SEM ) in 25 .
	manualset3
200640	15	417363	7	NULL	NULL	0	NULL	 25	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the mucosa close to the carcinoma of large bowel ( CLB ) in 200 cases , the carcinoma tissue of CLB in 130 and the mucosa of fetus large bowel in 24 by mucin histochemistry , in addition to the mucosa near CLB studied by scanning electron microscope ( SEM ) in 25 .
	manualset3
200641	1	417364	7	NULL	NULL	0	NULL	 relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the relationship between age and the iron-related signal loss on T2-weighted images in basal ganglia , and observed a strongly significant signal decrease in the globus pallidus at the age of brain development ( first two decades of life ) , but we found no such decrease in later years .
	manualset3
200642	2	417364	7	NULL	NULL	0	NULL	age	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the relationship between age and the iron-related signal loss on T2-weighted images in basal ganglia , and observed a strongly significant signal decrease in the globus pallidus at the age of brain development ( first two decades of life ) , but we found no such decrease in later years .
	manualset3
200643	3	417364	7	NULL	NULL	0	NULL	iron-related signal loss 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the relationship between age and the iron-related signal loss on T2-weighted images in basal ganglia , and observed a strongly significant signal decrease in the globus pallidus at the age of brain development ( first two decades of life ) , but we found no such decrease in later years .
	manualset3
200644	4	417364	7	NULL	NULL	0	NULL	T2-weighted images	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the relationship between age and the iron-related signal loss on T2-weighted images in basal ganglia , and observed a strongly significant signal decrease in the globus pallidus at the age of brain development ( first two decades of life ) , but we found no such decrease in later years .
	manualset3
200645	5	417364	7	NULL	NULL	0	NULL	basal ganglia	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the relationship between age and the iron-related signal loss on T2-weighted images in basal ganglia , and observed a strongly significant signal decrease in the globus pallidus at the age of brain development ( first two decades of life ) , but we found no such decrease in later years .
	manualset3
200646	6	417364	7	NULL	NULL	0	NULL	signal decrease	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the relationship between age and the iron-related signal loss on T2-weighted images in basal ganglia , and observed a strongly significant signal decrease in the globus pallidus at the age of brain development ( first two decades of life ) , but we found no such decrease in later years .
	manualset3
200647	7	417364	7	NULL	NULL	0	NULL	globus pallidus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the relationship between age and the iron-related signal loss on T2-weighted images in basal ganglia , and observed a strongly significant signal decrease in the globus pallidus at the age of brain development ( first two decades of life ) , but we found no such decrease in later years .
	manualset3
200648	8	417364	7	NULL	NULL	0	NULL	 age 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the relationship between age and the iron-related signal loss on T2-weighted images in basal ganglia , and observed a strongly significant signal decrease in the globus pallidus at the age of brain development ( first two decades of life ) , but we found no such decrease in later years .
	manualset3
200649	9	417364	7	NULL	NULL	0	NULL	brain development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the relationship between age and the iron-related signal loss on T2-weighted images in basal ganglia , and observed a strongly significant signal decrease in the globus pallidus at the age of brain development ( first two decades of life ) , but we found no such decrease in later years .
	manualset3
200650	10	417364	7	NULL	NULL	0	NULL	first two decades	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the relationship between age and the iron-related signal loss on T2-weighted images in basal ganglia , and observed a strongly significant signal decrease in the globus pallidus at the age of brain development ( first two decades of life ) , but we found no such decrease in later years .
	manualset3
200651	11	417364	7	NULL	NULL	0	NULL	 life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the relationship between age and the iron-related signal loss on T2-weighted images in basal ganglia , and observed a strongly significant signal decrease in the globus pallidus at the age of brain development ( first two decades of life ) , but we found no such decrease in later years .
	manualset3
200652	12	417364	7	NULL	NULL	0	NULL	decrease	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the relationship between age and the iron-related signal loss on T2-weighted images in basal ganglia , and observed a strongly significant signal decrease in the globus pallidus at the age of brain development ( first two decades of life ) , but we found no such decrease in later years .
	manualset3
200653	13	417364	7	NULL	NULL	0	NULL	later years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the relationship between age and the iron-related signal loss on T2-weighted images in basal ganglia , and observed a strongly significant signal decrease in the globus pallidus at the age of brain development ( first two decades of life ) , but we found no such decrease in later years .
	manualset3
200654	1	417365	7	NULL	NULL	0	NULL	relaxant effects 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the relaxant effects of OPC and mil on isolated human mesenteric arteries and veins in vitro .
	manualset3
200655	2	417365	7	NULL	NULL	0	NULL	OPC	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the relaxant effects of OPC and mil on isolated human mesenteric arteries and veins in vitro .
	manualset3
200656	3	417365	7	NULL	NULL	0	NULL	 mil	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the relaxant effects of OPC and mil on isolated human mesenteric arteries and veins in vitro .
	manualset3
200657	4	417365	7	NULL	NULL	0	NULL	isolated human mesenteric arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the relaxant effects of OPC and mil on isolated human mesenteric arteries and veins in vitro .
	manualset3
200658	5	417365	7	NULL	NULL	0	NULL	 isolated human mesenteric veins	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied the relaxant effects of OPC and mil on isolated human mesenteric arteries and veins in vitro .
	manualset3
200659	1	417366	7	NULL	NULL	0	NULL	pancreatic acinar cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied whether pancreatic acinar cells were also capable of responding to cytokines .
	manualset3
200660	2	417366	7	NULL	NULL	0	NULL	cytokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied whether pancreatic acinar cells were also capable of responding to cytokines .
	manualset3
200661	1	417367	7	NULL	NULL	0	NULL	system	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We study a system of grafted polymers in a poor solvent by self-consistent-field methods as well as Monte-Carlo simulation methods .
	manualset3
200662	2	417367	7	NULL	NULL	0	NULL	grafted polymers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We study a system of grafted polymers in a poor solvent by self-consistent-field methods as well as Monte-Carlo simulation methods .
	manualset3
200663	3	417367	7	NULL	NULL	0	NULL	poor solvent 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We study a system of grafted polymers in a poor solvent by self-consistent-field methods as well as Monte-Carlo simulation methods .
	manualset3
200664	4	417367	7	NULL	NULL	0	NULL	self-consistent-field methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We study a system of grafted polymers in a poor solvent by self-consistent-field methods as well as Monte-Carlo simulation methods .
	manualset3
200665	5	417367	7	NULL	NULL	0	NULL	Monte-Carlo simulation methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We study a system of grafted polymers in a poor solvent by self-consistent-field methods as well as Monte-Carlo simulation methods .
	manualset3
200666	1	417368	7	NULL	NULL	0	NULL	groups of membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	All groups of membranes were similar with respect to the rates of association and dissociation of hormone , degree of negative cooperativity and extents of both hormone and receptor inactivation .
	manualset3
200667	2	417368	7	NULL	NULL	0	NULL	rates of association	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All groups of membranes were similar with respect to the rates of association and dissociation of hormone , degree of negative cooperativity and extents of both hormone and receptor inactivation .
	manualset3
200668	3	417368	7	NULL	NULL	0	NULL	rates of dissociation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All groups of membranes were similar with respect to the rates of association and dissociation of hormone , degree of negative cooperativity and extents of both hormone and receptor inactivation .
	manualset3
200669	4	417368	7	NULL	NULL	NULL	NULL	 hormone	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	All groups of membranes were similar with respect to the rates of association and dissociation of hormone , degree of negative cooperativity and extents of both hormone and receptor inactivation .
	manualset3
200670	5	417368	7	NULL	NULL	0	NULL	degree	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All groups of membranes were similar with respect to the rates of association and dissociation of hormone , degree of negative cooperativity and extents of both hormone and receptor inactivation .
	manualset3
200671	6	417368	7	NULL	NULL	0	NULL	negative cooperativity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All groups of membranes were similar with respect to the rates of association and dissociation of hormone , degree of negative cooperativity and extents of both hormone and receptor inactivation .
	manualset3
200672	7	417368	7	NULL	NULL	0	NULL	extents	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All groups of membranes were similar with respect to the rates of association and dissociation of hormone , degree of negative cooperativity and extents of both hormone and receptor inactivation .
	manualset3
200673	8	417368	7	NULL	NULL	0	NULL	 hormone inactivation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All groups of membranes were similar with respect to the rates of association and dissociation of hormone , degree of negative cooperativity and extents of both hormone and receptor inactivation .
	manualset3
200674	9	417368	7	NULL	NULL	0	NULL	receptor inactivation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All groups of membranes were similar with respect to the rates of association and dissociation of hormone , degree of negative cooperativity and extents of both hormone and receptor inactivation .
	manualset3
200675	1	417369	7	NULL	NULL	0	NULL	renaturation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We study the renaturation of complementary single-stranded DNAs in a water-phenol two-phase system , with or without shaking .
	manualset3
200676	2	417369	7	NULL	NULL	0	NULL	complementary single-stranded DNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	We study the renaturation of complementary single-stranded DNAs in a water-phenol two-phase system , with or without shaking .
	manualset3
200677	3	417369	7	NULL	NULL	0	NULL	water-phenol two-phase system	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We study the renaturation of complementary single-stranded DNAs in a water-phenol two-phase system , with or without shaking .
	manualset3
200678	4	417369	7	NULL	NULL	0	NULL	shaking	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We study the renaturation of complementary single-stranded DNAs in a water-phenol two-phase system , with or without shaking .
	manualset3
200679	1	417370	7	NULL	NULL	0	NULL	binary system	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We study theoretically a binary system in which an attraction of unlike particles is combined with a type-independent soft-core repulsion .
	manualset3
200680	2	417370	7	NULL	NULL	0	NULL	attraction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We study theoretically a binary system in which an attraction of unlike particles is combined with a type-independent soft-core repulsion .
	manualset3
200681	3	417370	7	NULL	NULL	0	NULL	unlike particles	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	We study theoretically a binary system in which an attraction of unlike particles is combined with a type-independent soft-core repulsion .
	manualset3
200682	4	417370	7	NULL	NULL	0	NULL	type-independent soft-core repulsion	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We study theoretically a binary system in which an attraction of unlike particles is combined with a type-independent soft-core repulsion .
	manualset3
200683	1	417371	7	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest a model for the limb regeneration blastema where by 4 days post-amputation the blastema is already divided into distinct growth zones ; the cells of each zone are already specified to give rise to upper arm , lower arm , and hand .
	manualset3
200684	2	417371	7	NULL	NULL	0	NULL	limb regeneration blastema	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest a model for the limb regeneration blastema where by 4 days post-amputation the blastema is already divided into distinct growth zones ; the cells of each zone are already specified to give rise to upper arm , lower arm , and hand .
	manualset3
200685	3	417371	7	NULL	NULL	0	NULL	4 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest a model for the limb regeneration blastema where by 4 days post-amputation the blastema is already divided into distinct growth zones ; the cells of each zone are already specified to give rise to upper arm , lower arm , and hand .
	manualset3
200686	4	417371	7	NULL	NULL	NULL	NULL	post-amputation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We suggest a model for the limb regeneration blastema where by 4 days post-amputation the blastema is already divided into distinct growth zones ; the cells of each zone are already specified to give rise to upper arm , lower arm , and hand .
	manualset3
200687	5	417371	7	NULL	NULL	0	NULL	blastema	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest a model for the limb regeneration blastema where by 4 days post-amputation the blastema is already divided into distinct growth zones ; the cells of each zone are already specified to give rise to upper arm , lower arm , and hand .
	manualset3
200688	6	417371	7	NULL	NULL	0	NULL	distinct growth zones	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest a model for the limb regeneration blastema where by 4 days post-amputation the blastema is already divided into distinct growth zones ; the cells of each zone are already specified to give rise to upper arm , lower arm , and hand .
	manualset3
200689	7	417371	7	NULL	NULL	0	NULL	 cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest a model for the limb regeneration blastema where by 4 days post-amputation the blastema is already divided into distinct growth zones ; the cells of each zone are already specified to give rise to upper arm , lower arm , and hand .
	manualset3
200690	8	417371	7	NULL	NULL	0	NULL	 zone	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest a model for the limb regeneration blastema where by 4 days post-amputation the blastema is already divided into distinct growth zones ; the cells of each zone are already specified to give rise to upper arm , lower arm , and hand .
	manualset3
200691	9	417371	7	NULL	NULL	0	NULL	upper arm	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest a model for the limb regeneration blastema where by 4 days post-amputation the blastema is already divided into distinct growth zones ; the cells of each zone are already specified to give rise to upper arm , lower arm , and hand .
	manualset3
200692	10	417371	7	NULL	NULL	0	NULL	lower arm	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest a model for the limb regeneration blastema where by 4 days post-amputation the blastema is already divided into distinct growth zones ; the cells of each zone are already specified to give rise to upper arm , lower arm , and hand .
	manualset3
200693	11	417371	7	NULL	NULL	0	NULL	 hand 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest a model for the limb regeneration blastema where by 4 days post-amputation the blastema is already divided into distinct growth zones ; the cells of each zone are already specified to give rise to upper arm , lower arm , and hand .
	manualset3
200694	1	417372	7	NULL	NULL	0	NULL	uniform terminology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest a uniform terminology for this syndrome , either postpartum nephrosclerosis or nephrosclerosis in women taking oral contraceptives .
	manualset3
200695	2	417372	7	NULL	NULL	0	NULL	syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest a uniform terminology for this syndrome , either postpartum nephrosclerosis or nephrosclerosis in women taking oral contraceptives .
	manualset3
200696	3	417372	7	NULL	NULL	0	NULL	postpartum nephrosclerosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest a uniform terminology for this syndrome , either postpartum nephrosclerosis or nephrosclerosis in women taking oral contraceptives .
	manualset3
200697	4	417372	7	NULL	NULL	0	NULL	nephrosclerosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest a uniform terminology for this syndrome , either postpartum nephrosclerosis or nephrosclerosis in women taking oral contraceptives .
	manualset3
200698	5	417372	7	NULL	NULL	0	NULL	 women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest a uniform terminology for this syndrome , either postpartum nephrosclerosis or nephrosclerosis in women taking oral contraceptives .
	manualset3
200699	6	417372	7	NULL	NULL	0	NULL	oral contraceptives	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest a uniform terminology for this syndrome , either postpartum nephrosclerosis or nephrosclerosis in women taking oral contraceptives .
	manualset3
200700	1	417373	7	NULL	NULL	0	NULL	Tarasoff-type situation	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that , when faced with a Tarasoff-type situation , the appraisal of risk should be guided by a method that is primarily fact-based and deductive , rather than by the more inductive risk assessment approach for general violence recidivism , which is guided primarily by base rates and historical risk factors .
	manualset3
200701	2	417373	7	NULL	NULL	0	NULL	appraisal 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that , when faced with a Tarasoff-type situation , the appraisal of risk should be guided by a method that is primarily fact-based and deductive , rather than by the more inductive risk assessment approach for general violence recidivism , which is guided primarily by base rates and historical risk factors .
	manualset3
200702	3	417373	7	NULL	NULL	0	NULL	 risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that , when faced with a Tarasoff-type situation , the appraisal of risk should be guided by a method that is primarily fact-based and deductive , rather than by the more inductive risk assessment approach for general violence recidivism , which is guided primarily by base rates and historical risk factors .
	manualset3
200703	4	417373	7	NULL	NULL	0	NULL	method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that , when faced with a Tarasoff-type situation , the appraisal of risk should be guided by a method that is primarily fact-based and deductive , rather than by the more inductive risk assessment approach for general violence recidivism , which is guided primarily by base rates and historical risk factors .
	manualset3
200706	7	417373	7	NULL	NULL	0	NULL	inductive risk assessment approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that , when faced with a Tarasoff-type situation , the appraisal of risk should be guided by a method that is primarily fact-based and deductive , rather than by the more inductive risk assessment approach for general violence recidivism , which is guided primarily by base rates and historical risk factors .
	manualset3
200707	8	417373	7	NULL	NULL	0	NULL	general violence recidivism	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that , when faced with a Tarasoff-type situation , the appraisal of risk should be guided by a method that is primarily fact-based and deductive , rather than by the more inductive risk assessment approach for general violence recidivism , which is guided primarily by base rates and historical risk factors .
	manualset3
200708	9	417373	7	NULL	NULL	0	NULL	base rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that , when faced with a Tarasoff-type situation , the appraisal of risk should be guided by a method that is primarily fact-based and deductive , rather than by the more inductive risk assessment approach for general violence recidivism , which is guided primarily by base rates and historical risk factors .
	manualset3
200709	10	417373	7	NULL	NULL	0	NULL	historical risk factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that , when faced with a Tarasoff-type situation , the appraisal of risk should be guided by a method that is primarily fact-based and deductive , rather than by the more inductive risk assessment approach for general violence recidivism , which is guided primarily by base rates and historical risk factors .
	manualset3
200710	1	417374	7	NULL	NULL	0	NULL	CapD	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that CapD catalyses the capsule anchoring reaction .
	manualset3
200711	2	417374	7	NULL	NULL	0	NULL	capsule anchoring reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that CapD catalyses the capsule anchoring reaction .
	manualset3
200712	1	417375	7	NULL	NULL	0	NULL	DinB	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that DinB targets Pol III , thereby acting as a brake on replication fork progression .
	manualset3
200713	2	417375	7	NULL	NULL	0	NULL	Pol III	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that DinB targets Pol III , thereby acting as a brake on replication fork progression .
	manualset3
200714	3	417375	7	NULL	NULL	NULL	NULL	 brake	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We suggest that DinB targets Pol III , thereby acting as a brake on replication fork progression .
	manualset3
200715	4	417375	7	NULL	NULL	0	NULL	replication fork progression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that DinB targets Pol III , thereby acting as a brake on replication fork progression .
	manualset3
200716	1	417376	7	NULL	NULL	0	NULL	cleft palate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All had either a cleft palate and/or velopharyngeal incompetence , for which they underwent repair of the cleft palate or pharyngoplasty .
	manualset3
200717	2	417376	7	NULL	NULL	0	NULL	 velopharyngeal incompetence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All had either a cleft palate and/or velopharyngeal incompetence , for which they underwent repair of the cleft palate or pharyngoplasty .
	manualset3
200718	3	417376	7	NULL	NULL	0	NULL	repair	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All had either a cleft palate and/or velopharyngeal incompetence , for which they underwent repair of the cleft palate or pharyngoplasty .
	manualset3
200719	4	417376	7	NULL	NULL	0	NULL	cleft palate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All had either a cleft palate and/or velopharyngeal incompetence , for which they underwent repair of the cleft palate or pharyngoplasty .
	manualset3
200720	5	417376	7	NULL	NULL	0	NULL	pharyngoplasty	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All had either a cleft palate and/or velopharyngeal incompetence , for which they underwent repair of the cleft palate or pharyngoplasty .
	manualset3
200721	1	417377	7	NULL	NULL	0	NULL	N-cadherin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that N-cadherin acts primarily in the adhesion between glial cells during postnatal development .
	manualset3
200722	2	417377	7	NULL	NULL	0	NULL	adhesion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that N-cadherin acts primarily in the adhesion between glial cells during postnatal development .
	manualset3
200723	3	417377	7	NULL	NULL	0	NULL	glial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that N-cadherin acts primarily in the adhesion between glial cells during postnatal development .
	manualset3
200724	4	417377	7	NULL	NULL	0	NULL	postnatal development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that N-cadherin acts primarily in the adhesion between glial cells during postnatal development .
	manualset3
200725	1	417378	7	NULL	NULL	0	NULL	aberrant expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that aberrant expression and interactions of betaIII-tubulin and gamma-tubulin may be linked to malignant changes in glial cells .
	manualset3
200726	2	417378	7	NULL	NULL	0	NULL	 interactions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that aberrant expression and interactions of betaIII-tubulin and gamma-tubulin may be linked to malignant changes in glial cells .
	manualset3
200727	3	417378	7	NULL	NULL	0	NULL	betaIII-tubulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that aberrant expression and interactions of betaIII-tubulin and gamma-tubulin may be linked to malignant changes in glial cells .
	manualset3
200728	4	417378	7	NULL	NULL	0	NULL	gamma-tubulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that aberrant expression and interactions of betaIII-tubulin and gamma-tubulin may be linked to malignant changes in glial cells .
	manualset3
200729	5	417378	7	NULL	NULL	0	NULL	malignant changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that aberrant expression and interactions of betaIII-tubulin and gamma-tubulin may be linked to malignant changes in glial cells .
	manualset3
200730	6	417378	7	NULL	NULL	0	NULL	glial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that aberrant expression and interactions of betaIII-tubulin and gamma-tubulin may be linked to malignant changes in glial cells .
	manualset3
200731	1	417379	7	NULL	NULL	0	NULL	hyperthyroidism	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that hyperthyroidism be included in the differential diagnosis of PH .
	manualset3
200732	2	417379	7	NULL	NULL	0	NULL	 differential diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that hyperthyroidism be included in the differential diagnosis of PH .
	manualset3
200733	3	417379	7	NULL	NULL	0	NULL	PH	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that hyperthyroidism be included in the differential diagnosis of PH .
	manualset3
200734	1	417380	7	NULL	NULL	0	NULL	 intragastric lipolysis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that intragastric lipolysis is probably of major importance in the newborn and especially in the premature infant where it compensates not only for low pancreatic lipase , but in addition , helps to overcome the temporary bile salt deficiency through the formation of amphiphilic reaction products .
	manualset3
200735	2	417380	7	NULL	NULL	0	NULL	newborn	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that intragastric lipolysis is probably of major importance in the newborn and especially in the premature infant where it compensates not only for low pancreatic lipase , but in addition , helps to overcome the temporary bile salt deficiency through the formation of amphiphilic reaction products .
	manualset3
200736	3	417380	7	NULL	NULL	0	NULL	premature infant	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that intragastric lipolysis is probably of major importance in the newborn and especially in the premature infant where it compensates not only for low pancreatic lipase , but in addition , helps to overcome the temporary bile salt deficiency through the formation of amphiphilic reaction products .
	manualset3
200737	4	417380	7	NULL	NULL	0	NULL	low pancreatic lipase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that intragastric lipolysis is probably of major importance in the newborn and especially in the premature infant where it compensates not only for low pancreatic lipase , but in addition , helps to overcome the temporary bile salt deficiency through the formation of amphiphilic reaction products .
	manualset3
200738	5	417380	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that intragastric lipolysis is probably of major importance in the newborn and especially in the premature infant where it compensates not only for low pancreatic lipase , but in addition , helps to overcome the temporary bile salt deficiency through the formation of amphiphilic reaction products .
	manualset3
200739	6	417380	7	NULL	NULL	0	NULL	 temporary bile salt deficiency 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that intragastric lipolysis is probably of major importance in the newborn and especially in the premature infant where it compensates not only for low pancreatic lipase , but in addition , helps to overcome the temporary bile salt deficiency through the formation of amphiphilic reaction products .
	manualset3
200740	7	417380	7	NULL	NULL	0	NULL	 formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that intragastric lipolysis is probably of major importance in the newborn and especially in the premature infant where it compensates not only for low pancreatic lipase , but in addition , helps to overcome the temporary bile salt deficiency through the formation of amphiphilic reaction products .
	manualset3
200741	8	417380	7	NULL	NULL	0	NULL	amphiphilic reaction products	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that intragastric lipolysis is probably of major importance in the newborn and especially in the premature infant where it compensates not only for low pancreatic lipase , but in addition , helps to overcome the temporary bile salt deficiency through the formation of amphiphilic reaction products .
	manualset3
200742	1	417381	7	NULL	NULL	0	NULL	placenta-derived cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that placenta-derived cells have multilineage differentiation potential similar to MSCs in terms of morphology and cell-surface antigen expression .
	manualset3
200743	2	417381	7	NULL	NULL	0	NULL	multilineage differentiation potential	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that placenta-derived cells have multilineage differentiation potential similar to MSCs in terms of morphology and cell-surface antigen expression .
	manualset3
200744	3	417381	7	NULL	NULL	0	NULL	MSCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that placenta-derived cells have multilineage differentiation potential similar to MSCs in terms of morphology and cell-surface antigen expression .
	manualset3
200745	4	417381	7	NULL	NULL	0	NULL	morphology 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that placenta-derived cells have multilineage differentiation potential similar to MSCs in terms of morphology and cell-surface antigen expression .
	manualset3
200746	5	417381	7	NULL	NULL	0	NULL	cell-surface antigen expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that placenta-derived cells have multilineage differentiation potential similar to MSCs in terms of morphology and cell-surface antigen expression .
	manualset3
200747	1	417382	7	NULL	NULL	0	NULL	protein kinase C 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that protein kinase C can both prevent the decay of the high activity state and convert the low activity state into the high activity state .
	manualset3
200748	2	417382	7	NULL	NULL	0	NULL	 decay	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that protein kinase C can both prevent the decay of the high activity state and convert the low activity state into the high activity state .
	manualset3
200749	3	417382	7	NULL	NULL	0	NULL	high activity state	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that protein kinase C can both prevent the decay of the high activity state and convert the low activity state into the high activity state .
	manualset3
200750	4	417382	7	NULL	NULL	0	NULL	low activity state	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that protein kinase C can both prevent the decay of the high activity state and convert the low activity state into the high activity state .
	manualset3
200751	5	417382	7	NULL	NULL	0	NULL	high activity state	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that protein kinase C can both prevent the decay of the high activity state and convert the low activity state into the high activity state .
	manualset3
200752	1	417383	7	NULL	NULL	0	NULL	carcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that some carcinomas of the lung with the light-microscopic and cytologic appearance of small cell anaplastic carcinoma are actually small cell variants of squamous cell carcinoma and lack the characteristic neurosecretory granules of classic small cell carcinoma .
	manualset3
200753	2	417383	7	NULL	NULL	0	NULL	 lung	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that some carcinomas of the lung with the light-microscopic and cytologic appearance of small cell anaplastic carcinoma are actually small cell variants of squamous cell carcinoma and lack the characteristic neurosecretory granules of classic small cell carcinoma .
	manualset3
200754	3	417383	7	NULL	NULL	0	NULL	 light-microscopic appearance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that some carcinomas of the lung with the light-microscopic and cytologic appearance of small cell anaplastic carcinoma are actually small cell variants of squamous cell carcinoma and lack the characteristic neurosecretory granules of classic small cell carcinoma .
	manualset3
200755	4	417383	7	NULL	NULL	0	NULL	cytologic appearance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that some carcinomas of the lung with the light-microscopic and cytologic appearance of small cell anaplastic carcinoma are actually small cell variants of squamous cell carcinoma and lack the characteristic neurosecretory granules of classic small cell carcinoma .
	manualset3
200756	5	417383	7	NULL	NULL	0	NULL	small cell anaplastic carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that some carcinomas of the lung with the light-microscopic and cytologic appearance of small cell anaplastic carcinoma are actually small cell variants of squamous cell carcinoma and lack the characteristic neurosecretory granules of classic small cell carcinoma .
	manualset3
200757	6	417383	7	NULL	NULL	0	NULL	small cell variants	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that some carcinomas of the lung with the light-microscopic and cytologic appearance of small cell anaplastic carcinoma are actually small cell variants of squamous cell carcinoma and lack the characteristic neurosecretory granules of classic small cell carcinoma .
	manualset3
200758	7	417383	7	NULL	NULL	0	NULL	squamous cell carcinoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that some carcinomas of the lung with the light-microscopic and cytologic appearance of small cell anaplastic carcinoma are actually small cell variants of squamous cell carcinoma and lack the characteristic neurosecretory granules of classic small cell carcinoma .
	manualset3
200759	8	417383	7	NULL	NULL	0	NULL	neurosecretory granules	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that some carcinomas of the lung with the light-microscopic and cytologic appearance of small cell anaplastic carcinoma are actually small cell variants of squamous cell carcinoma and lack the characteristic neurosecretory granules of classic small cell carcinoma .
	manualset3
200760	9	417383	7	NULL	NULL	0	NULL	classic small cell carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that some carcinomas of the lung with the light-microscopic and cytologic appearance of small cell anaplastic carcinoma are actually small cell variants of squamous cell carcinoma and lack the characteristic neurosecretory granules of classic small cell carcinoma .
	manualset3
200761	1	417384	7	NULL	NULL	0	NULL	chromosomal operon	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the chromosomal operon is the primarily expressed copy and the plasmid operon acts as a backup to maintain appropriate gene dosages .
	manualset3
200762	2	417384	7	NULL	NULL	NULL	NULL	 plasmid operon 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We suggest that the chromosomal operon is the primarily expressed copy and the plasmid operon acts as a backup to maintain appropriate gene dosages .
	manualset3
200763	3	417384	7	NULL	NULL	0	NULL	gene dosages	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the chromosomal operon is the primarily expressed copy and the plasmid operon acts as a backup to maintain appropriate gene dosages .
	manualset3
200764	4	417384	7	NULL	NULL	0	NULL	copy	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the chromosomal operon is the primarily expressed copy and the plasmid operon acts as a backup to maintain appropriate gene dosages .
	manualset3
200765	1	417385	7	NULL	NULL	0	NULL	cytoplasmic region 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the cytoplasmic region containing the WR may be responsible for their difference in solubility .
	manualset3
200766	2	417385	7	NULL	NULL	0	NULL	WR	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the cytoplasmic region containing the WR may be responsible for their difference in solubility .
	manualset3
200767	3	417385	7	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the cytoplasmic region containing the WR may be responsible for their difference in solubility .
	manualset3
200768	4	417385	7	NULL	NULL	0	NULL	solubility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the cytoplasmic region containing the WR may be responsible for their difference in solubility .
	manualset3
200769	1	417386	7	NULL	NULL	0	NULL	 protein-creatinine ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the protein-creatinine ratio in random urine samples could replace the timed collection methods at least for follow-up and screening .
	manualset3
200770	2	417386	7	NULL	NULL	0	NULL	random urine samples	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the protein-creatinine ratio in random urine samples could replace the timed collection methods at least for follow-up and screening .
	manualset3
200771	3	417386	7	NULL	NULL	0	NULL	timed collection methods	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the protein-creatinine ratio in random urine samples could replace the timed collection methods at least for follow-up and screening .
	manualset3
200772	4	417386	7	NULL	NULL	0	NULL	follow-up	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the protein-creatinine ratio in random urine samples could replace the timed collection methods at least for follow-up and screening .
	manualset3
200773	5	417386	7	NULL	NULL	0	NULL	screening	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the protein-creatinine ratio in random urine samples could replace the timed collection methods at least for follow-up and screening .
	manualset3
200774	1	417387	7	NULL	NULL	0	NULL	skin lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the skin lesions observed in our patient represent an unusual response to ultraviolet damage to melanocytes followed by reactive epidermal hyperkeratosis .
	manualset3
200775	2	417387	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the skin lesions observed in our patient represent an unusual response to ultraviolet damage to melanocytes followed by reactive epidermal hyperkeratosis .
	manualset3
200776	3	417387	7	NULL	NULL	0	NULL	unusual response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the skin lesions observed in our patient represent an unusual response to ultraviolet damage to melanocytes followed by reactive epidermal hyperkeratosis .
	manualset3
200777	4	417387	7	NULL	NULL	0	NULL	ultraviolet damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the skin lesions observed in our patient represent an unusual response to ultraviolet damage to melanocytes followed by reactive epidermal hyperkeratosis .
	manualset3
200778	5	417387	7	NULL	NULL	0	NULL	melanocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the skin lesions observed in our patient represent an unusual response to ultraviolet damage to melanocytes followed by reactive epidermal hyperkeratosis .
	manualset3
200779	6	417387	7	NULL	NULL	0	NULL	reactive epidermal hyperkeratosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the skin lesions observed in our patient represent an unusual response to ultraviolet damage to melanocytes followed by reactive epidermal hyperkeratosis .
	manualset3
200780	1	417388	7	NULL	NULL	0	NULL	sources of signals	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the sources of signals that specify hippocampal field identity lie close to the hippocampal poles , and that the signals operate first on cells at the poles , then move inwards .
	manualset3
200781	2	417388	7	NULL	NULL	0	NULL	hippocampal field identity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the sources of signals that specify hippocampal field identity lie close to the hippocampal poles , and that the signals operate first on cells at the poles , then move inwards .
	manualset3
200782	3	417388	7	NULL	NULL	0	NULL	hippocampal poles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the sources of signals that specify hippocampal field identity lie close to the hippocampal poles , and that the signals operate first on cells at the poles , then move inwards .
	manualset3
200783	4	417388	7	NULL	NULL	0	NULL	signals	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the sources of signals that specify hippocampal field identity lie close to the hippocampal poles , and that the signals operate first on cells at the poles , then move inwards .
	manualset3
200784	5	417388	7	NULL	NULL	0	NULL	 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the sources of signals that specify hippocampal field identity lie close to the hippocampal poles , and that the signals operate first on cells at the poles , then move inwards .
	manualset3
200785	6	417388	7	NULL	NULL	0	NULL	 poles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the sources of signals that specify hippocampal field identity lie close to the hippocampal poles , and that the signals operate first on cells at the poles , then move inwards .
	manualset3
200786	1	417389	7	NULL	NULL	0	NULL	 voltage sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the voltage sensitivity of both the ionic conductance of the channel seen at the highest salt concentration and its blockage by the crown reflects a field-induced deformation of the pore .
	manualset3
200787	2	417389	7	NULL	NULL	0	NULL	 ionic conductance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the voltage sensitivity of both the ionic conductance of the channel seen at the highest salt concentration and its blockage by the crown reflects a field-induced deformation of the pore .
	manualset3
200788	3	417389	7	NULL	NULL	0	NULL	 channel	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the voltage sensitivity of both the ionic conductance of the channel seen at the highest salt concentration and its blockage by the crown reflects a field-induced deformation of the pore .
	manualset3
200789	4	417389	7	NULL	NULL	0	NULL	highest salt concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the voltage sensitivity of both the ionic conductance of the channel seen at the highest salt concentration and its blockage by the crown reflects a field-induced deformation of the pore .
	manualset3
200790	5	417389	7	NULL	NULL	0	NULL	blockage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the voltage sensitivity of both the ionic conductance of the channel seen at the highest salt concentration and its blockage by the crown reflects a field-induced deformation of the pore .
	manualset3
200791	6	417389	7	NULL	NULL	NULL	NULL	 crown	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We suggest that the voltage sensitivity of both the ionic conductance of the channel seen at the highest salt concentration and its blockage by the crown reflects a field-induced deformation of the pore .
	manualset3
200792	7	417389	7	NULL	NULL	0	NULL	 field-induced deformation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the voltage sensitivity of both the ionic conductance of the channel seen at the highest salt concentration and its blockage by the crown reflects a field-induced deformation of the pore .
	manualset3
200793	8	417389	7	NULL	NULL	0	NULL	pore	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the voltage sensitivity of both the ionic conductance of the channel seen at the highest salt concentration and its blockage by the crown reflects a field-induced deformation of the pore .
	manualset3
200794	1	417390	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	We summarize here the data presented at a workshop on CH , at which factors potentially related to the CH-incidence-rate increase ( namely , race , ethnicity , sex , and birth outcomes ) were evaluated .
	manualset3
200795	2	417390	7	NULL	NULL	0	NULL	workshop	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	We summarize here the data presented at a workshop on CH , at which factors potentially related to the CH-incidence-rate increase ( namely , race , ethnicity , sex , and birth outcomes ) were evaluated .
	manualset3
200796	3	417390	7	NULL	NULL	0	NULL	CH	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We summarize here the data presented at a workshop on CH , at which factors potentially related to the CH-incidence-rate increase ( namely , race , ethnicity , sex , and birth outcomes ) were evaluated .
	manualset3
200797	4	417390	7	NULL	NULL	0	NULL	factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We summarize here the data presented at a workshop on CH , at which factors potentially related to the CH-incidence-rate increase ( namely , race , ethnicity , sex , and birth outcomes ) were evaluated .
	manualset3
200798	5	417390	7	NULL	NULL	0	NULL	 CH-incidence-rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We summarize here the data presented at a workshop on CH , at which factors potentially related to the CH-incidence-rate increase ( namely , race , ethnicity , sex , and birth outcomes ) were evaluated .
	manualset3
200799	6	417390	7	NULL	NULL	0	NULL	race	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We summarize here the data presented at a workshop on CH , at which factors potentially related to the CH-incidence-rate increase ( namely , race , ethnicity , sex , and birth outcomes ) were evaluated .
	manualset3
200800	7	417390	7	NULL	NULL	0	NULL	 ethnicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We summarize here the data presented at a workshop on CH , at which factors potentially related to the CH-incidence-rate increase ( namely , race , ethnicity , sex , and birth outcomes ) were evaluated .
	manualset3
200801	8	417390	7	NULL	NULL	0	NULL	sex	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We summarize here the data presented at a workshop on CH , at which factors potentially related to the CH-incidence-rate increase ( namely , race , ethnicity , sex , and birth outcomes ) were evaluated .
	manualset3
200802	9	417390	7	NULL	NULL	0	NULL	birth outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We summarize here the data presented at a workshop on CH , at which factors potentially related to the CH-incidence-rate increase ( namely , race , ethnicity , sex , and birth outcomes ) were evaluated .
	manualset3
200803	1	417391	7	NULL	NULL	NULL	NULL	tendency	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We suppressed the tendency of Aequorea fluorescent proteins to dimerize and targeted these variants to the plasma membrane using several different types of lipid anchors .
	manualset3
200804	2	417391	7	NULL	NULL	0	NULL	Aequorea fluorescent proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We suppressed the tendency of Aequorea fluorescent proteins to dimerize and targeted these variants to the plasma membrane using several different types of lipid anchors .
	manualset3
200805	3	417391	7	NULL	NULL	0	NULL	variants 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	We suppressed the tendency of Aequorea fluorescent proteins to dimerize and targeted these variants to the plasma membrane using several different types of lipid anchors .
	manualset3
200806	4	417391	7	NULL	NULL	0	NULL	plasma membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	We suppressed the tendency of Aequorea fluorescent proteins to dimerize and targeted these variants to the plasma membrane using several different types of lipid anchors .
	manualset3
200807	5	417391	7	NULL	NULL	0	NULL	different types	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We suppressed the tendency of Aequorea fluorescent proteins to dimerize and targeted these variants to the plasma membrane using several different types of lipid anchors .
	manualset3
200808	6	417391	7	NULL	NULL	0	NULL	lipid anchors	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We suppressed the tendency of Aequorea fluorescent proteins to dimerize and targeted these variants to the plasma membrane using several different types of lipid anchors .
	manualset3
200809	1	417392	7	NULL	NULL	0	NULL	1 , 540 physicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We surveyed 1 , 540 physicians from four specialty groups ( cardiologists , surgeons , obstetrician-gynecologists , and internists ) using specialty-specific clinical scenarios .
	manualset3
200810	2	417392	7	NULL	NULL	0	NULL	four specialty groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We surveyed 1 , 540 physicians from four specialty groups ( cardiologists , surgeons , obstetrician-gynecologists , and internists ) using specialty-specific clinical scenarios .
	manualset3
200811	3	417392	7	NULL	NULL	0	NULL	cardiologists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We surveyed 1 , 540 physicians from four specialty groups ( cardiologists , surgeons , obstetrician-gynecologists , and internists ) using specialty-specific clinical scenarios .
	manualset3
200812	4	417392	7	NULL	NULL	0	NULL	surgeons	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We surveyed 1 , 540 physicians from four specialty groups ( cardiologists , surgeons , obstetrician-gynecologists , and internists ) using specialty-specific clinical scenarios .
	manualset3
200813	5	417392	7	NULL	NULL	0	NULL	obstetrician-gynecologists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We surveyed 1 , 540 physicians from four specialty groups ( cardiologists , surgeons , obstetrician-gynecologists , and internists ) using specialty-specific clinical scenarios .
	manualset3
200814	6	417392	7	NULL	NULL	0	NULL	 internists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We surveyed 1 , 540 physicians from four specialty groups ( cardiologists , surgeons , obstetrician-gynecologists , and internists ) using specialty-specific clinical scenarios .
	manualset3
200815	7	417392	7	NULL	NULL	0	NULL	specialty-specific clinical scenarios	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We surveyed 1 , 540 physicians from four specialty groups ( cardiologists , surgeons , obstetrician-gynecologists , and internists ) using specialty-specific clinical scenarios .
	manualset3
200816	1	417393	7	NULL	NULL	0	NULL	gene shuffling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested an alternative to gene shuffling based on plasmid recombination and found that Bacillus subtilis efficiently recombines sequences with 4 % divergence , and Escherichia coli mutS is more appropriate for sequences with 22 % divergence .
	manualset3
200817	2	417393	7	NULL	NULL	0	NULL	plasmid recombination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested an alternative to gene shuffling based on plasmid recombination and found that Bacillus subtilis efficiently recombines sequences with 4 % divergence , and Escherichia coli mutS is more appropriate for sequences with 22 % divergence .
	manualset3
200818	3	417393	7	NULL	NULL	0	NULL	Bacillus subtilis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested an alternative to gene shuffling based on plasmid recombination and found that Bacillus subtilis efficiently recombines sequences with 4 % divergence , and Escherichia coli mutS is more appropriate for sequences with 22 % divergence .
	manualset3
200819	4	417393	7	NULL	NULL	0	NULL	sequences	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested an alternative to gene shuffling based on plasmid recombination and found that Bacillus subtilis efficiently recombines sequences with 4 % divergence , and Escherichia coli mutS is more appropriate for sequences with 22 % divergence .
	manualset3
200820	5	417393	7	NULL	NULL	0	NULL	 4 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested an alternative to gene shuffling based on plasmid recombination and found that Bacillus subtilis efficiently recombines sequences with 4 % divergence , and Escherichia coli mutS is more appropriate for sequences with 22 % divergence .
	manualset3
200821	6	417393	7	NULL	NULL	0	NULL	divergence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested an alternative to gene shuffling based on plasmid recombination and found that Bacillus subtilis efficiently recombines sequences with 4 % divergence , and Escherichia coli mutS is more appropriate for sequences with 22 % divergence .
	manualset3
200822	7	417393	7	NULL	NULL	0	NULL	Escherichia coli mutS	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested an alternative to gene shuffling based on plasmid recombination and found that Bacillus subtilis efficiently recombines sequences with 4 % divergence , and Escherichia coli mutS is more appropriate for sequences with 22 % divergence .
	manualset3
200823	8	417393	7	NULL	NULL	0	NULL	sequences 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested an alternative to gene shuffling based on plasmid recombination and found that Bacillus subtilis efficiently recombines sequences with 4 % divergence , and Escherichia coli mutS is more appropriate for sequences with 22 % divergence .
	manualset3
200824	9	417393	7	NULL	NULL	0	NULL	22 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested an alternative to gene shuffling based on plasmid recombination and found that Bacillus subtilis efficiently recombines sequences with 4 % divergence , and Escherichia coli mutS is more appropriate for sequences with 22 % divergence .
	manualset3
200825	10	417393	7	NULL	NULL	0	NULL	divergence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested an alternative to gene shuffling based on plasmid recombination and found that Bacillus subtilis efficiently recombines sequences with 4 % divergence , and Escherichia coli mutS is more appropriate for sequences with 22 % divergence .
	manualset3
200826	1	417394	7	NULL	NULL	0	NULL	 effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the effects of various types of fatty acids , differing in the degree of saturation and in the cis/trans configuration of the double bond , on the growth and viability of NES2Y cells ( a human pancreatic beta-cell line ) .
	manualset3
200827	2	417394	7	NULL	NULL	0	NULL	various types	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the effects of various types of fatty acids , differing in the degree of saturation and in the cis/trans configuration of the double bond , on the growth and viability of NES2Y cells ( a human pancreatic beta-cell line ) .
	manualset3
200828	3	417394	7	NULL	NULL	0	NULL	fatty acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the effects of various types of fatty acids , differing in the degree of saturation and in the cis/trans configuration of the double bond , on the growth and viability of NES2Y cells ( a human pancreatic beta-cell line ) .
	manualset3
200829	4	417394	7	NULL	NULL	0	NULL	degree of saturation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the effects of various types of fatty acids , differing in the degree of saturation and in the cis/trans configuration of the double bond , on the growth and viability of NES2Y cells ( a human pancreatic beta-cell line ) .
	manualset3
200830	5	417394	7	NULL	NULL	0	NULL	cis/trans configuration	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the effects of various types of fatty acids , differing in the degree of saturation and in the cis/trans configuration of the double bond , on the growth and viability of NES2Y cells ( a human pancreatic beta-cell line ) .
	manualset3
200831	6	417394	7	NULL	NULL	0	NULL	double bond	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the effects of various types of fatty acids , differing in the degree of saturation and in the cis/trans configuration of the double bond , on the growth and viability of NES2Y cells ( a human pancreatic beta-cell line ) .
	manualset3
200832	7	417394	7	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the effects of various types of fatty acids , differing in the degree of saturation and in the cis/trans configuration of the double bond , on the growth and viability of NES2Y cells ( a human pancreatic beta-cell line ) .
	manualset3
200833	8	417394	7	NULL	NULL	0	NULL	viability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the effects of various types of fatty acids , differing in the degree of saturation and in the cis/trans configuration of the double bond , on the growth and viability of NES2Y cells ( a human pancreatic beta-cell line ) .
	manualset3
200834	9	417394	7	NULL	NULL	0	NULL	NES2Y cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the effects of various types of fatty acids , differing in the degree of saturation and in the cis/trans configuration of the double bond , on the growth and viability of NES2Y cells ( a human pancreatic beta-cell line ) .
	manualset3
200835	10	417394	7	NULL	NULL	0	NULL	human pancreatic beta-cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the effects of various types of fatty acids , differing in the degree of saturation and in the cis/trans configuration of the double bond , on the growth and viability of NES2Y cells ( a human pancreatic beta-cell line ) .
	manualset3
200836	1	417395	7	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All had had three or more stone events .
	manualset3
200837	2	417395	7	NULL	NULL	0	NULL	stone events	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	All had had three or more stone events .
	manualset3
200838	1	417396	7	NULL	NULL	0	NULL	 hypothesis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the hypothesis that Ang II infusion results in an elevation of uPA expression contributing to aneurysm formation .
	manualset3
200839	2	417396	7	NULL	NULL	NULL	NULL	Ang II infusion	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We tested the hypothesis that Ang II infusion results in an elevation of uPA expression contributing to aneurysm formation .
	manualset3
200840	3	417396	7	NULL	NULL	0	NULL	 elevation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the hypothesis that Ang II infusion results in an elevation of uPA expression contributing to aneurysm formation .
	manualset3
200841	4	417396	7	NULL	NULL	0	NULL	uPA expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the hypothesis that Ang II infusion results in an elevation of uPA expression contributing to aneurysm formation .
	manualset3
200842	5	417396	7	NULL	NULL	0	NULL	aneurysm formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the hypothesis that Ang II infusion results in an elevation of uPA expression contributing to aneurysm formation .
	manualset3
200843	1	417397	7	NULL	NULL	0	NULL	hypothesis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the hypothesis that changes in the subcellular distribution of the proapoptotic protein Bax precede the activation of downstream apoptosis-effector mechanisms such as caspase-3 cleavage and endonuclease activation during the progression of excitotoxic neuronal apoptosis in the striatum of newborn rat .
	manualset3
200844	2	417397	7	NULL	NULL	0	NULL	changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the hypothesis that changes in the subcellular distribution of the proapoptotic protein Bax precede the activation of downstream apoptosis-effector mechanisms such as caspase-3 cleavage and endonuclease activation during the progression of excitotoxic neuronal apoptosis in the striatum of newborn rat .
	manualset3
200845	3	417397	7	NULL	NULL	0	NULL	 subcellular distribution 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the hypothesis that changes in the subcellular distribution of the proapoptotic protein Bax precede the activation of downstream apoptosis-effector mechanisms such as caspase-3 cleavage and endonuclease activation during the progression of excitotoxic neuronal apoptosis in the striatum of newborn rat .
	manualset3
200846	4	417397	7	NULL	NULL	0	NULL	 proapoptotic protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the hypothesis that changes in the subcellular distribution of the proapoptotic protein Bax precede the activation of downstream apoptosis-effector mechanisms such as caspase-3 cleavage and endonuclease activation during the progression of excitotoxic neuronal apoptosis in the striatum of newborn rat .
	manualset3
200847	5	417397	7	NULL	NULL	0	NULL	Bax	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the hypothesis that changes in the subcellular distribution of the proapoptotic protein Bax precede the activation of downstream apoptosis-effector mechanisms such as caspase-3 cleavage and endonuclease activation during the progression of excitotoxic neuronal apoptosis in the striatum of newborn rat .
	manualset3
200848	6	417397	7	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the hypothesis that changes in the subcellular distribution of the proapoptotic protein Bax precede the activation of downstream apoptosis-effector mechanisms such as caspase-3 cleavage and endonuclease activation during the progression of excitotoxic neuronal apoptosis in the striatum of newborn rat .
	manualset3
200849	7	417397	7	NULL	NULL	0	NULL	downstream apoptosis-effector mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the hypothesis that changes in the subcellular distribution of the proapoptotic protein Bax precede the activation of downstream apoptosis-effector mechanisms such as caspase-3 cleavage and endonuclease activation during the progression of excitotoxic neuronal apoptosis in the striatum of newborn rat .
	manualset3
200850	8	417397	7	NULL	NULL	0	NULL	caspase-3 cleavage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the hypothesis that changes in the subcellular distribution of the proapoptotic protein Bax precede the activation of downstream apoptosis-effector mechanisms such as caspase-3 cleavage and endonuclease activation during the progression of excitotoxic neuronal apoptosis in the striatum of newborn rat .
	manualset3
200851	9	417397	7	NULL	NULL	0	NULL	endonuclease activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the hypothesis that changes in the subcellular distribution of the proapoptotic protein Bax precede the activation of downstream apoptosis-effector mechanisms such as caspase-3 cleavage and endonuclease activation during the progression of excitotoxic neuronal apoptosis in the striatum of newborn rat .
	manualset3
200852	10	417397	7	NULL	NULL	0	NULL	progression 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the hypothesis that changes in the subcellular distribution of the proapoptotic protein Bax precede the activation of downstream apoptosis-effector mechanisms such as caspase-3 cleavage and endonuclease activation during the progression of excitotoxic neuronal apoptosis in the striatum of newborn rat .
	manualset3
200853	11	417397	7	NULL	NULL	0	NULL	excitotoxic neuronal apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the hypothesis that changes in the subcellular distribution of the proapoptotic protein Bax precede the activation of downstream apoptosis-effector mechanisms such as caspase-3 cleavage and endonuclease activation during the progression of excitotoxic neuronal apoptosis in the striatum of newborn rat .
	manualset3
200854	12	417397	7	NULL	NULL	0	NULL	 striatum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the hypothesis that changes in the subcellular distribution of the proapoptotic protein Bax precede the activation of downstream apoptosis-effector mechanisms such as caspase-3 cleavage and endonuclease activation during the progression of excitotoxic neuronal apoptosis in the striatum of newborn rat .
	manualset3
200855	13	417397	7	NULL	NULL	0	NULL	newborn rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the hypothesis that changes in the subcellular distribution of the proapoptotic protein Bax precede the activation of downstream apoptosis-effector mechanisms such as caspase-3 cleavage and endonuclease activation during the progression of excitotoxic neuronal apoptosis in the striatum of newborn rat .
	manualset3
200856	1	417398	7	NULL	NULL	0	NULL	hypothesis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the hypothesis that enkephalins or some other compound ( s ) released by the adrenal medulla during hemorrhage were responsible for the resultant hypotension .
	manualset3
200857	2	417398	7	NULL	NULL	0	NULL	enkephalins	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the hypothesis that enkephalins or some other compound ( s ) released by the adrenal medulla during hemorrhage were responsible for the resultant hypotension .
	manualset3
200858	3	417398	7	NULL	NULL	0	NULL	compound ( s )	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the hypothesis that enkephalins or some other compound ( s ) released by the adrenal medulla during hemorrhage were responsible for the resultant hypotension .
	manualset3
200859	4	417398	7	NULL	NULL	0	NULL	adrenal medulla	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the hypothesis that enkephalins or some other compound ( s ) released by the adrenal medulla during hemorrhage were responsible for the resultant hypotension .
	manualset3
200860	5	417398	7	NULL	NULL	0	NULL	hemorrhage 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the hypothesis that enkephalins or some other compound ( s ) released by the adrenal medulla during hemorrhage were responsible for the resultant hypotension .
	manualset3
200861	6	417398	7	NULL	NULL	0	NULL	resultant hypotension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the hypothesis that enkephalins or some other compound ( s ) released by the adrenal medulla during hemorrhage were responsible for the resultant hypotension .
	manualset3
200862	1	417399	7	NULL	NULL	0	NULL	hypothesis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the hypothesis that the mitogen-activated protein kinases ( MAPK ) form transducers for the damaging effects of high glucose .
	manualset3
200863	2	417399	7	NULL	NULL	NULL	NULL	mitogen-activated protein kinases ( MAPK )	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We tested the hypothesis that the mitogen-activated protein kinases ( MAPK ) form transducers for the damaging effects of high glucose .
	manualset3
200864	3	417399	7	NULL	NULL	NULL	NULL	transducers	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We tested the hypothesis that the mitogen-activated protein kinases ( MAPK ) form transducers for the damaging effects of high glucose .
	manualset3
200865	4	417399	7	NULL	NULL	0	NULL	damaging effects 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the hypothesis that the mitogen-activated protein kinases ( MAPK ) form transducers for the damaging effects of high glucose .
	manualset3
200866	5	417399	7	NULL	NULL	NULL	NULL	high glucose	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We tested the hypothesis that the mitogen-activated protein kinases ( MAPK ) form transducers for the damaging effects of high glucose .
	manualset3
200867	1	417400	7	NULL	NULL	0	NULL	short-term efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the short-term efficacy and feasibility of two stress education approaches toe the treatment of mild hypertension in older African Americans .
	manualset3
200868	2	417400	7	NULL	NULL	0	NULL	 feasibility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the short-term efficacy and feasibility of two stress education approaches toe the treatment of mild hypertension in older African Americans .
	manualset3
200869	3	417400	7	NULL	NULL	0	NULL	 two stress education approaches	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the short-term efficacy and feasibility of two stress education approaches toe the treatment of mild hypertension in older African Americans .
	manualset3
200870	4	417400	7	NULL	NULL	0	NULL	 treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the short-term efficacy and feasibility of two stress education approaches toe the treatment of mild hypertension in older African Americans .
	manualset3
200871	5	417400	7	NULL	NULL	0	NULL	mild hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the short-term efficacy and feasibility of two stress education approaches toe the treatment of mild hypertension in older African Americans .
	manualset3
200872	6	417400	7	NULL	NULL	0	NULL	older African Americans	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested the short-term efficacy and feasibility of two stress education approaches toe the treatment of mild hypertension in older African Americans .
	manualset3
200873	1	417401	7	NULL	NULL	0	NULL	hypothesis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested this hypothesis by analyzing Mbd4 - / - mice and found that the frequency of of C -- ) T transitions at CpG sites was increased by a factor of three .
	manualset3
200874	2	417401	7	NULL	NULL	0	NULL	Mbd4 - / - mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested this hypothesis by analyzing Mbd4 - / - mice and found that the frequency of of C -- ) T transitions at CpG sites was increased by a factor of three .
	manualset3
200875	3	417401	7	NULL	NULL	0	NULL	frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested this hypothesis by analyzing Mbd4 - / - mice and found that the frequency of of C -- ) T transitions at CpG sites was increased by a factor of three .
	manualset3
200876	4	417401	7	NULL	NULL	0	NULL	C -- ) T transitions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested this hypothesis by analyzing Mbd4 - / - mice and found that the frequency of of C -- ) T transitions at CpG sites was increased by a factor of three .
	manualset3
200877	5	417401	7	NULL	NULL	0	NULL	CpG sites	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested this hypothesis by analyzing Mbd4 - / - mice and found that the frequency of of C -- ) T transitions at CpG sites was increased by a factor of three .
	manualset3
200878	6	417401	7	NULL	NULL	0	NULL	 factor	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested this hypothesis by analyzing Mbd4 - / - mice and found that the frequency of of C -- ) T transitions at CpG sites was increased by a factor of three .
	manualset3
200879	7	417401	7	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested this hypothesis by analyzing Mbd4 - / - mice and found that the frequency of of C -- ) T transitions at CpG sites was increased by a factor of three .
	manualset3
200880	1	417402	7	NULL	NULL	0	NULL	position	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested this position by examining the relationship between cardiorespiratory fitness and N-acetylaspartate ( NAA ) levels in the right frontal cortex using magnetic resonance spectroscopy .
	manualset3
200881	2	417402	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested this position by examining the relationship between cardiorespiratory fitness and N-acetylaspartate ( NAA ) levels in the right frontal cortex using magnetic resonance spectroscopy .
	manualset3
200882	3	417402	7	NULL	NULL	0	NULL	cardiorespiratory fitness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested this position by examining the relationship between cardiorespiratory fitness and N-acetylaspartate ( NAA ) levels in the right frontal cortex using magnetic resonance spectroscopy .
	manualset3
200883	4	417402	7	NULL	NULL	0	NULL	N-acetylaspartate ( NAA ) levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested this position by examining the relationship between cardiorespiratory fitness and N-acetylaspartate ( NAA ) levels in the right frontal cortex using magnetic resonance spectroscopy .
	manualset3
200884	5	417402	7	NULL	NULL	0	NULL	right frontal cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested this position by examining the relationship between cardiorespiratory fitness and N-acetylaspartate ( NAA ) levels in the right frontal cortex using magnetic resonance spectroscopy .
	manualset3
200885	6	417402	7	NULL	NULL	0	NULL	magnetic resonance spectroscopy 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested this position by examining the relationship between cardiorespiratory fitness and N-acetylaspartate ( NAA ) levels in the right frontal cortex using magnetic resonance spectroscopy .
	manualset3
200886	1	417403	7	NULL	NULL	0	NULL	small-molecule	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested whether the small-molecule and orphan drug dichloroacetate ( DCA ) can reverse this cancer-specific metabolic and mitochondrial remodeling in glioblastoma .
	manualset3
200887	2	417403	7	NULL	NULL	0	NULL	orphan drug dichloroacetate ( DCA )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested whether the small-molecule and orphan drug dichloroacetate ( DCA ) can reverse this cancer-specific metabolic and mitochondrial remodeling in glioblastoma .
	manualset3
200888	3	417403	7	NULL	NULL	0	NULL	cancer-specific metabolic remodeling 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested whether the small-molecule and orphan drug dichloroacetate ( DCA ) can reverse this cancer-specific metabolic and mitochondrial remodeling in glioblastoma .
	manualset3
200889	4	417403	7	NULL	NULL	0	NULL	mitochondrial remodeling	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested whether the small-molecule and orphan drug dichloroacetate ( DCA ) can reverse this cancer-specific metabolic and mitochondrial remodeling in glioblastoma .
	manualset3
200890	5	417403	7	NULL	NULL	0	NULL	glioblastoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We tested whether the small-molecule and orphan drug dichloroacetate ( DCA ) can reverse this cancer-specific metabolic and mitochondrial remodeling in glioblastoma .
	manualset3
200891	1	417404	7	NULL	NULL	0	NULL	anti-inflammatory activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All have anti-inflammatory and analgesic activity and all can cause gastrointestinal side effects , though effectiveness and toxicity vary from drug to drug and patient to patient , there being very great interpatient variability .
	manualset3
200892	2	417404	7	NULL	NULL	0	NULL	analgesic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All have anti-inflammatory and analgesic activity and all can cause gastrointestinal side effects , though effectiveness and toxicity vary from drug to drug and patient to patient , there being very great interpatient variability .
	manualset3
200893	3	417404	7	NULL	NULL	0	NULL	gastrointestinal side effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All have anti-inflammatory and analgesic activity and all can cause gastrointestinal side effects , though effectiveness and toxicity vary from drug to drug and patient to patient , there being very great interpatient variability .
	manualset3
200894	4	417404	7	NULL	NULL	0	NULL	effectiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All have anti-inflammatory and analgesic activity and all can cause gastrointestinal side effects , though effectiveness and toxicity vary from drug to drug and patient to patient , there being very great interpatient variability .
	manualset3
200895	5	417404	7	NULL	NULL	0	NULL	toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All have anti-inflammatory and analgesic activity and all can cause gastrointestinal side effects , though effectiveness and toxicity vary from drug to drug and patient to patient , there being very great interpatient variability .
	manualset3
200896	6	417404	7	NULL	NULL	0	NULL	drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	All have anti-inflammatory and analgesic activity and all can cause gastrointestinal side effects , though effectiveness and toxicity vary from drug to drug and patient to patient , there being very great interpatient variability .
	manualset3
200897	7	417404	7	NULL	NULL	0	NULL	 drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	All have anti-inflammatory and analgesic activity and all can cause gastrointestinal side effects , though effectiveness and toxicity vary from drug to drug and patient to patient , there being very great interpatient variability .
	manualset3
200898	8	417404	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	All have anti-inflammatory and analgesic activity and all can cause gastrointestinal side effects , though effectiveness and toxicity vary from drug to drug and patient to patient , there being very great interpatient variability .
	manualset3
200899	9	417404	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	All have anti-inflammatory and analgesic activity and all can cause gastrointestinal side effects , though effectiveness and toxicity vary from drug to drug and patient to patient , there being very great interpatient variability .
	manualset3
200900	10	417404	7	NULL	NULL	0	NULL	interpatient variability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	All have anti-inflammatory and analgesic activity and all can cause gastrointestinal side effects , though effectiveness and toxicity vary from drug to drug and patient to patient , there being very great interpatient variability .
	manualset3
200901	1	417405	7	NULL	NULL	0	NULL	antigen matched , LM-specific CD8 + T cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We then generate antigen matched , LM-specific CD8 + T cell lines from wild-type and gene knockout mice , and compare their capacity to provide immunity to LM infection in vivo .
	manualset3
200902	2	417405	7	NULL	NULL	0	NULL	wild-type mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We then generate antigen matched , LM-specific CD8 + T cell lines from wild-type and gene knockout mice , and compare their capacity to provide immunity to LM infection in vivo .
	manualset3
200903	3	417405	7	NULL	NULL	0	NULL	gene knockout mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We then generate antigen matched , LM-specific CD8 + T cell lines from wild-type and gene knockout mice , and compare their capacity to provide immunity to LM infection in vivo .
	manualset3
200904	4	417405	7	NULL	NULL	NULL	NULL	capacity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We then generate antigen matched , LM-specific CD8 + T cell lines from wild-type and gene knockout mice , and compare their capacity to provide immunity to LM infection in vivo .
	manualset3
200905	5	417405	7	NULL	NULL	0	NULL	immunity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We then generate antigen matched , LM-specific CD8 + T cell lines from wild-type and gene knockout mice , and compare their capacity to provide immunity to LM infection in vivo .
	manualset3
200906	6	417405	7	NULL	NULL	0	NULL	LM infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We then generate antigen matched , LM-specific CD8 + T cell lines from wild-type and gene knockout mice , and compare their capacity to provide immunity to LM infection in vivo .
	manualset3
200928	1	417406	7	NULL	NULL	0	NULL	`` simulation '' capability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We then introduce a `` simulation '' capability , such that the robot has an internal representation of its interaction with the world .
	manualset3
200929	2	417406	7	NULL	NULL	0	NULL	robot	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We then introduce a `` simulation '' capability , such that the robot has an internal representation of its interaction with the world .
	manualset3
200930	3	417406	7	NULL	NULL	0	NULL	internal representation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We then introduce a `` simulation '' capability , such that the robot has an internal representation of its interaction with the world .
	manualset3
200931	4	417406	7	NULL	NULL	0	NULL	interaction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We then introduce a `` simulation '' capability , such that the robot has an internal representation of its interaction with the world .
	manualset3
200932	5	417406	7	NULL	NULL	0	NULL	world	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	We then introduce a `` simulation '' capability , such that the robot has an internal representation of its interaction with the world .
	manualset3
200933	1	417407	7	NULL	NULL	0	NULL	effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We then investigated the effects of leptin produced by BM adipocytes on APL cells using a coculture system with mesenchymal stem cell ( MSC ) - derived adipocytes .
	manualset3
200934	2	417407	7	NULL	NULL	0	NULL	leptin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We then investigated the effects of leptin produced by BM adipocytes on APL cells using a coculture system with mesenchymal stem cell ( MSC ) - derived adipocytes .
	manualset3
200935	3	417407	7	NULL	NULL	0	NULL	BM adipocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We then investigated the effects of leptin produced by BM adipocytes on APL cells using a coculture system with mesenchymal stem cell ( MSC ) - derived adipocytes .
	manualset3
200936	4	417407	7	NULL	NULL	0	NULL	APL cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We then investigated the effects of leptin produced by BM adipocytes on APL cells using a coculture system with mesenchymal stem cell ( MSC ) - derived adipocytes .
	manualset3
200937	5	417407	7	NULL	NULL	0	NULL	 coculture system 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We then investigated the effects of leptin produced by BM adipocytes on APL cells using a coculture system with mesenchymal stem cell ( MSC ) - derived adipocytes .
	manualset3
200938	6	417407	7	NULL	NULL	0	NULL	mesenchymal stem cell ( MSC ) - derived adipocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We then investigated the effects of leptin produced by BM adipocytes on APL cells using a coculture system with mesenchymal stem cell ( MSC ) - derived adipocytes .
	manualset3
200939	1	417408	7	NULL	NULL	0	NULL	acyl-CoA synthetase 1 ( ACSL1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore investigated whether acyl-CoA synthetase 1 ( ACSL1 ) , a key enzyme mediating acyl-CoA synthesis in macrophages , could directly influence ABCA1 levels and cholesterol efflux in these cells .
	manualset3
200940	2	417408	7	NULL	NULL	0	NULL	 key enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore investigated whether acyl-CoA synthetase 1 ( ACSL1 ) , a key enzyme mediating acyl-CoA synthesis in macrophages , could directly influence ABCA1 levels and cholesterol efflux in these cells .
	manualset3
200941	3	417408	7	NULL	NULL	0	NULL	acyl-CoA synthesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore investigated whether acyl-CoA synthetase 1 ( ACSL1 ) , a key enzyme mediating acyl-CoA synthesis in macrophages , could directly influence ABCA1 levels and cholesterol efflux in these cells .
	manualset3
200942	4	417408	7	NULL	NULL	0	NULL	macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore investigated whether acyl-CoA synthetase 1 ( ACSL1 ) , a key enzyme mediating acyl-CoA synthesis in macrophages , could directly influence ABCA1 levels and cholesterol efflux in these cells .
	manualset3
200943	5	417408	7	NULL	NULL	0	NULL	ABCA1 levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore investigated whether acyl-CoA synthetase 1 ( ACSL1 ) , a key enzyme mediating acyl-CoA synthesis in macrophages , could directly influence ABCA1 levels and cholesterol efflux in these cells .
	manualset3
200945	6	417408	7	NULL	NULL	0	NULL	cholesterol efflux	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore investigated whether acyl-CoA synthetase 1 ( ACSL1 ) , a key enzyme mediating acyl-CoA synthesis in macrophages , could directly influence ABCA1 levels and cholesterol efflux in these cells .
	manualset3
200946	7	417408	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore investigated whether acyl-CoA synthetase 1 ( ACSL1 ) , a key enzyme mediating acyl-CoA synthesis in macrophages , could directly influence ABCA1 levels and cholesterol efflux in these cells .
	manualset3
200947	1	417409	7	NULL	NULL	0	NULL	hydroxyl group	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore propose that the hydroxyl group of Tyr-60 participates in a hydrogen bond that is important for the initial complex formation with IGF-I and the stabilization of this complex .
	manualset3
200948	2	417409	7	NULL	NULL	0	NULL	Tyr-60 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore propose that the hydroxyl group of Tyr-60 participates in a hydrogen bond that is important for the initial complex formation with IGF-I and the stabilization of this complex .
	manualset3
200949	3	417409	7	NULL	NULL	0	NULL	hydrogen bond 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore propose that the hydroxyl group of Tyr-60 participates in a hydrogen bond that is important for the initial complex formation with IGF-I and the stabilization of this complex .
	manualset3
200950	4	417409	7	NULL	NULL	0	NULL	initial complex formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore propose that the hydroxyl group of Tyr-60 participates in a hydrogen bond that is important for the initial complex formation with IGF-I and the stabilization of this complex .
	manualset3
200951	5	417409	7	NULL	NULL	0	NULL	IGF-I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore propose that the hydroxyl group of Tyr-60 participates in a hydrogen bond that is important for the initial complex formation with IGF-I and the stabilization of this complex .
	manualset3
200952	6	417409	7	NULL	NULL	0	NULL	 stabilization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore propose that the hydroxyl group of Tyr-60 participates in a hydrogen bond that is important for the initial complex formation with IGF-I and the stabilization of this complex .
	manualset3
200953	7	417409	7	NULL	NULL	0	NULL	complex	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore propose that the hydroxyl group of Tyr-60 participates in a hydrogen bond that is important for the initial complex formation with IGF-I and the stabilization of this complex .
	manualset3
200954	1	417410	7	NULL	NULL	0	NULL	hsm mutants	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	All hsm mutants were resistant to the lethal effect of these mutagens .
	manualset3
200955	2	417410	7	NULL	NULL	0	NULL	lethal effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All hsm mutants were resistant to the lethal effect of these mutagens .
	manualset3
200956	3	417410	7	NULL	NULL	0	NULL	mutagens	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All hsm mutants were resistant to the lethal effect of these mutagens .
	manualset3
200957	1	417411	7	NULL	NULL	0	NULL	OASIS protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore proposed that OASIS protein positively regulated gene transcription in a subset of reactive astrocytes , and thereby influenced the reaction of injured CNS tissues .
	manualset3
200958	2	417411	7	NULL	NULL	0	NULL	gene transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore proposed that OASIS protein positively regulated gene transcription in a subset of reactive astrocytes , and thereby influenced the reaction of injured CNS tissues .
	manualset3
200959	3	417411	7	NULL	NULL	0	NULL	subset	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore proposed that OASIS protein positively regulated gene transcription in a subset of reactive astrocytes , and thereby influenced the reaction of injured CNS tissues .
	manualset3
200960	4	417411	7	NULL	NULL	0	NULL	 reactive astrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore proposed that OASIS protein positively regulated gene transcription in a subset of reactive astrocytes , and thereby influenced the reaction of injured CNS tissues .
	manualset3
200961	5	417411	7	NULL	NULL	0	NULL	reaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore proposed that OASIS protein positively regulated gene transcription in a subset of reactive astrocytes , and thereby influenced the reaction of injured CNS tissues .
	manualset3
200962	6	417411	7	NULL	NULL	0	NULL	injured CNS tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore proposed that OASIS protein positively regulated gene transcription in a subset of reactive astrocytes , and thereby influenced the reaction of injured CNS tissues .
	manualset3
200963	1	417412	7	NULL	NULL	0	NULL	chloroplast genome ( cpDNA )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore sequenced the entire chloroplast genome ( cpDNA ) of Phalaenopsis aphrodite , Taiwan moth orchid .
	manualset3
200964	2	417412	7	NULL	NULL	0	NULL	Phalaenopsis aphrodite	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore sequenced the entire chloroplast genome ( cpDNA ) of Phalaenopsis aphrodite , Taiwan moth orchid .
	manualset3
200965	3	417412	7	NULL	NULL	0	NULL	 Taiwan moth orchid	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore sequenced the entire chloroplast genome ( cpDNA ) of Phalaenopsis aphrodite , Taiwan moth orchid .
	manualset3
200966	1	417413	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore sought evidence for human leucocyte antigen ( HLA ) restriction and variant frequency differences in selected polymorphisms at the loci for the immunomodulatory cytokines , tumor necrosis factor alpha ( TNF-alpha ) , lymphotoxin-alpha ( LT-alpha ) and interleukin 10 ( IL-10 ) in patients with MDS and acute myeloid leukemia ( AML ) compared with normal controls .
	manualset3
200967	2	417413	7	NULL	NULL	NULL	NULL	human leucocyte antigen ( HLA ) restriction	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We therefore sought evidence for human leucocyte antigen ( HLA ) restriction and variant frequency differences in selected polymorphisms at the loci for the immunomodulatory cytokines , tumor necrosis factor alpha ( TNF-alpha ) , lymphotoxin-alpha ( LT-alpha ) and interleukin 10 ( IL-10 ) in patients with MDS and acute myeloid leukemia ( AML ) compared with normal controls .
	manualset3
200968	3	417413	7	NULL	NULL	0	NULL	variant frequency differences 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore sought evidence for human leucocyte antigen ( HLA ) restriction and variant frequency differences in selected polymorphisms at the loci for the immunomodulatory cytokines , tumor necrosis factor alpha ( TNF-alpha ) , lymphotoxin-alpha ( LT-alpha ) and interleukin 10 ( IL-10 ) in patients with MDS and acute myeloid leukemia ( AML ) compared with normal controls .
	manualset3
200969	4	417413	7	NULL	NULL	0	NULL	selected polymorphisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore sought evidence for human leucocyte antigen ( HLA ) restriction and variant frequency differences in selected polymorphisms at the loci for the immunomodulatory cytokines , tumor necrosis factor alpha ( TNF-alpha ) , lymphotoxin-alpha ( LT-alpha ) and interleukin 10 ( IL-10 ) in patients with MDS and acute myeloid leukemia ( AML ) compared with normal controls .
	manualset3
200970	5	417413	7	NULL	NULL	0	NULL	loci	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore sought evidence for human leucocyte antigen ( HLA ) restriction and variant frequency differences in selected polymorphisms at the loci for the immunomodulatory cytokines , tumor necrosis factor alpha ( TNF-alpha ) , lymphotoxin-alpha ( LT-alpha ) and interleukin 10 ( IL-10 ) in patients with MDS and acute myeloid leukemia ( AML ) compared with normal controls .
	manualset3
200971	6	417413	7	NULL	NULL	0	NULL	immunomodulatory cytokines 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore sought evidence for human leucocyte antigen ( HLA ) restriction and variant frequency differences in selected polymorphisms at the loci for the immunomodulatory cytokines , tumor necrosis factor alpha ( TNF-alpha ) , lymphotoxin-alpha ( LT-alpha ) and interleukin 10 ( IL-10 ) in patients with MDS and acute myeloid leukemia ( AML ) compared with normal controls .
	manualset3
200972	7	417413	7	NULL	NULL	0	NULL	tumor necrosis factor alpha ( TNF-alpha )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore sought evidence for human leucocyte antigen ( HLA ) restriction and variant frequency differences in selected polymorphisms at the loci for the immunomodulatory cytokines , tumor necrosis factor alpha ( TNF-alpha ) , lymphotoxin-alpha ( LT-alpha ) and interleukin 10 ( IL-10 ) in patients with MDS and acute myeloid leukemia ( AML ) compared with normal controls .
	manualset3
200973	8	417413	7	NULL	NULL	0	NULL	 lymphotoxin-alpha ( LT-alpha )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore sought evidence for human leucocyte antigen ( HLA ) restriction and variant frequency differences in selected polymorphisms at the loci for the immunomodulatory cytokines , tumor necrosis factor alpha ( TNF-alpha ) , lymphotoxin-alpha ( LT-alpha ) and interleukin 10 ( IL-10 ) in patients with MDS and acute myeloid leukemia ( AML ) compared with normal controls .
	manualset3
200974	9	417413	7	NULL	NULL	0	NULL	interleukin 10 ( IL-10 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore sought evidence for human leucocyte antigen ( HLA ) restriction and variant frequency differences in selected polymorphisms at the loci for the immunomodulatory cytokines , tumor necrosis factor alpha ( TNF-alpha ) , lymphotoxin-alpha ( LT-alpha ) and interleukin 10 ( IL-10 ) in patients with MDS and acute myeloid leukemia ( AML ) compared with normal controls .
	manualset3
200975	10	417413	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore sought evidence for human leucocyte antigen ( HLA ) restriction and variant frequency differences in selected polymorphisms at the loci for the immunomodulatory cytokines , tumor necrosis factor alpha ( TNF-alpha ) , lymphotoxin-alpha ( LT-alpha ) and interleukin 10 ( IL-10 ) in patients with MDS and acute myeloid leukemia ( AML ) compared with normal controls .
	manualset3
200976	11	417413	7	NULL	NULL	0	NULL	MDS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore sought evidence for human leucocyte antigen ( HLA ) restriction and variant frequency differences in selected polymorphisms at the loci for the immunomodulatory cytokines , tumor necrosis factor alpha ( TNF-alpha ) , lymphotoxin-alpha ( LT-alpha ) and interleukin 10 ( IL-10 ) in patients with MDS and acute myeloid leukemia ( AML ) compared with normal controls .
	manualset3
200977	12	417413	7	NULL	NULL	0	NULL	acute myeloid leukemia ( AML ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore sought evidence for human leucocyte antigen ( HLA ) restriction and variant frequency differences in selected polymorphisms at the loci for the immunomodulatory cytokines , tumor necrosis factor alpha ( TNF-alpha ) , lymphotoxin-alpha ( LT-alpha ) and interleukin 10 ( IL-10 ) in patients with MDS and acute myeloid leukemia ( AML ) compared with normal controls .
	manualset3
200978	13	417413	7	NULL	NULL	0	NULL	normal controls .	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore sought evidence for human leucocyte antigen ( HLA ) restriction and variant frequency differences in selected polymorphisms at the loci for the immunomodulatory cytokines , tumor necrosis factor alpha ( TNF-alpha ) , lymphotoxin-alpha ( LT-alpha ) and interleukin 10 ( IL-10 ) in patients with MDS and acute myeloid leukemia ( AML ) compared with normal controls .
	manualset3
200979	1	417414	7	NULL	NULL	0	NULL	business modeling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore suggest that business modeling can be used as an effective approach to supporting holistic development of eHealth technologies .
	manualset3
200980	2	417414	7	NULL	NULL	0	NULL	effective approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore suggest that business modeling can be used as an effective approach to supporting holistic development of eHealth technologies .
	manualset3
200981	3	417414	7	NULL	NULL	0	NULL	holistic development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore suggest that business modeling can be used as an effective approach to supporting holistic development of eHealth technologies .
	manualset3
200982	4	417414	7	NULL	NULL	0	NULL	eHealth technologies	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore suggest that business modeling can be used as an effective approach to supporting holistic development of eHealth technologies .
	manualset3
200983	1	417415	7	NULL	NULL	0	NULL	environmental factors 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We think that environmental factors could be more important than genetic factors in the arousal of cardiovascular diseases .
	manualset3
200984	2	417415	7	NULL	NULL	0	NULL	genetic factors	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	We think that environmental factors could be more important than genetic factors in the arousal of cardiovascular diseases .
	manualset3
200985	3	417415	7	NULL	NULL	0	NULL	 arousal	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We think that environmental factors could be more important than genetic factors in the arousal of cardiovascular diseases .
	manualset3
200986	4	417415	7	NULL	NULL	0	NULL	cardiovascular diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We think that environmental factors could be more important than genetic factors in the arousal of cardiovascular diseases .
	manualset3
201007	1	417416	7	NULL	NULL	0	NULL	 differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	We thus analyzed the differences in the structures , dynamics , and energy surfaces of the protein in its soluble state or in situations where it aggregates through conformational states that have native-like structure , folding stability , and enzymatic activity .
	manualset3
201008	2	417416	7	NULL	NULL	0	NULL	 structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We thus analyzed the differences in the structures , dynamics , and energy surfaces of the protein in its soluble state or in situations where it aggregates through conformational states that have native-like structure , folding stability , and enzymatic activity .
	manualset3
201011	3	417416	7	NULL	NULL	0	NULL	dynamics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We thus analyzed the differences in the structures , dynamics , and energy surfaces of the protein in its soluble state or in situations where it aggregates through conformational states that have native-like structure , folding stability , and enzymatic activity .
	manualset3
201012	4	417416	7	NULL	NULL	0	NULL	energy surfaces	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We thus analyzed the differences in the structures , dynamics , and energy surfaces of the protein in its soluble state or in situations where it aggregates through conformational states that have native-like structure , folding stability , and enzymatic activity .
	manualset3
201013	5	417416	7	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We thus analyzed the differences in the structures , dynamics , and energy surfaces of the protein in its soluble state or in situations where it aggregates through conformational states that have native-like structure , folding stability , and enzymatic activity .
	manualset3
201014	6	417416	7	NULL	NULL	NULL	NULL	soluble state	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We thus analyzed the differences in the structures , dynamics , and energy surfaces of the protein in its soluble state or in situations where it aggregates through conformational states that have native-like structure , folding stability , and enzymatic activity .
	manualset3
201015	7	417416	7	NULL	NULL	0	NULL	situations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We thus analyzed the differences in the structures , dynamics , and energy surfaces of the protein in its soluble state or in situations where it aggregates through conformational states that have native-like structure , folding stability , and enzymatic activity .
	manualset3
201016	8	417416	7	NULL	NULL	0	NULL	conformational states	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We thus analyzed the differences in the structures , dynamics , and energy surfaces of the protein in its soluble state or in situations where it aggregates through conformational states that have native-like structure , folding stability , and enzymatic activity .
	manualset3
201017	9	417416	7	NULL	NULL	0	NULL	native-like structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We thus analyzed the differences in the structures , dynamics , and energy surfaces of the protein in its soluble state or in situations where it aggregates through conformational states that have native-like structure , folding stability , and enzymatic activity .
	manualset3
201018	10	417416	7	NULL	NULL	0	NULL	folding stability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We thus analyzed the differences in the structures , dynamics , and energy surfaces of the protein in its soluble state or in situations where it aggregates through conformational states that have native-like structure , folding stability , and enzymatic activity .
	manualset3
201019	11	417416	7	NULL	NULL	0	NULL	enzymatic activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We thus analyzed the differences in the structures , dynamics , and energy surfaces of the protein in its soluble state or in situations where it aggregates through conformational states that have native-like structure , folding stability , and enzymatic activity .
	manualset3
201020	1	417417	7	NULL	NULL	0	NULL	ecological study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We undertook an ecological study to investigate differences in coronary heart disease mortality within Nottingham health authority , England , to establish whether coronary mortality varied according to socio-economic status , and how mortality rates changed over a decade .
	manualset3
201021	2	417417	7	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	We undertook an ecological study to investigate differences in coronary heart disease mortality within Nottingham health authority , England , to establish whether coronary mortality varied according to socio-economic status , and how mortality rates changed over a decade .
	manualset3
201022	3	417417	7	NULL	NULL	0	NULL	coronary heart disease mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We undertook an ecological study to investigate differences in coronary heart disease mortality within Nottingham health authority , England , to establish whether coronary mortality varied according to socio-economic status , and how mortality rates changed over a decade .
	manualset3
201023	4	417417	7	NULL	NULL	0	NULL	Nottingham health authority	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	We undertook an ecological study to investigate differences in coronary heart disease mortality within Nottingham health authority , England , to establish whether coronary mortality varied according to socio-economic status , and how mortality rates changed over a decade .
	manualset3
201024	5	417417	7	NULL	NULL	0	NULL	England	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	We undertook an ecological study to investigate differences in coronary heart disease mortality within Nottingham health authority , England , to establish whether coronary mortality varied according to socio-economic status , and how mortality rates changed over a decade .
	manualset3
201025	6	417417	7	NULL	NULL	0	NULL	coronary mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We undertook an ecological study to investigate differences in coronary heart disease mortality within Nottingham health authority , England , to establish whether coronary mortality varied according to socio-economic status , and how mortality rates changed over a decade .
	manualset3
201026	7	417417	7	NULL	NULL	0	NULL	socio-economic status	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We undertook an ecological study to investigate differences in coronary heart disease mortality within Nottingham health authority , England , to establish whether coronary mortality varied according to socio-economic status , and how mortality rates changed over a decade .
	manualset3
201027	8	417417	7	NULL	NULL	0	NULL	mortality rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We undertook an ecological study to investigate differences in coronary heart disease mortality within Nottingham health authority , England , to establish whether coronary mortality varied according to socio-economic status , and how mortality rates changed over a decade .
	manualset3
201028	9	417417	7	NULL	NULL	0	NULL	decade 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	We undertook an ecological study to investigate differences in coronary heart disease mortality within Nottingham health authority , England , to establish whether coronary mortality varied according to socio-economic status , and how mortality rates changed over a decade .
	manualset3
201029	1	417418	7	NULL	NULL	0	NULL	basin-hopping global optimization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We use basin-hopping global optimization to identify the most stable structures for the A ( 1-42 ) peptide monomer and small oligomers up to the octamer inserted into a lipid bilayer .
	manualset3
201030	2	417418	7	NULL	NULL	0	NULL	stable structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We use basin-hopping global optimization to identify the most stable structures for the A ( 1-42 ) peptide monomer and small oligomers up to the octamer inserted into a lipid bilayer .
	manualset3
201031	3	417418	7	NULL	NULL	0	NULL	A ( 1-42 ) peptide monomer	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	We use basin-hopping global optimization to identify the most stable structures for the A ( 1-42 ) peptide monomer and small oligomers up to the octamer inserted into a lipid bilayer .
	manualset3
201032	4	417418	7	NULL	NULL	0	NULL	small oligomers	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	We use basin-hopping global optimization to identify the most stable structures for the A ( 1-42 ) peptide monomer and small oligomers up to the octamer inserted into a lipid bilayer .
	manualset3
201033	5	417418	7	NULL	NULL	0	NULL	octamer	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	We use basin-hopping global optimization to identify the most stable structures for the A ( 1-42 ) peptide monomer and small oligomers up to the octamer inserted into a lipid bilayer .
	manualset3
201034	6	417418	7	NULL	NULL	0	NULL	lipid bilayer	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We use basin-hopping global optimization to identify the most stable structures for the A ( 1-42 ) peptide monomer and small oligomers up to the octamer inserted into a lipid bilayer .
	manualset3
201037	1	417419	7	NULL	NULL	0	NULL	human subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All human subjects in this study were trained to localize short bursts of noise in a darkened anechoic environment .
	manualset3
201039	2	417419	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	All human subjects in this study were trained to localize short bursts of noise in a darkened anechoic environment .
	manualset3
201041	3	417419	7	NULL	NULL	0	NULL	short bursts of noise	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	All human subjects in this study were trained to localize short bursts of noise in a darkened anechoic environment .
	manualset3
201043	4	417419	7	NULL	NULL	0	NULL	 darkened anechoic environment	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	All human subjects in this study were trained to localize short bursts of noise in a darkened anechoic environment .
	manualset3
201044	1	417420	7	NULL	NULL	0	NULL	 instrument 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	We use the instrument to quantitatively monitor rapid changes in refractive index within defined subregions of cells due to exposure to acetic acid or changes in medium osmolarity .
	manualset3
201045	2	417420	7	NULL	NULL	0	NULL	 rapid changes 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We use the instrument to quantitatively monitor rapid changes in refractive index within defined subregions of cells due to exposure to acetic acid or changes in medium osmolarity .
	manualset3
201046	3	417420	7	NULL	NULL	0	NULL	refractive index	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We use the instrument to quantitatively monitor rapid changes in refractive index within defined subregions of cells due to exposure to acetic acid or changes in medium osmolarity .
	manualset3
201047	4	417420	7	NULL	NULL	0	NULL	subregions of cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We use the instrument to quantitatively monitor rapid changes in refractive index within defined subregions of cells due to exposure to acetic acid or changes in medium osmolarity .
	manualset3
201048	5	417420	7	NULL	NULL	0	NULL	acetic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We use the instrument to quantitatively monitor rapid changes in refractive index within defined subregions of cells due to exposure to acetic acid or changes in medium osmolarity .
	manualset3
201049	6	417420	7	NULL	NULL	0	NULL	 changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We use the instrument to quantitatively monitor rapid changes in refractive index within defined subregions of cells due to exposure to acetic acid or changes in medium osmolarity .
	manualset3
201050	7	417420	7	NULL	NULL	0	NULL	medium osmolarity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We use the instrument to quantitatively monitor rapid changes in refractive index within defined subregions of cells due to exposure to acetic acid or changes in medium osmolarity .
	manualset3
201052	1	417421	7	NULL	NULL	0	NULL	genus-level phylogeny	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	We used a genus-level phylogeny ( nuclear marker , ETS2 ) , which included several taxa from all other acanthurid genera , to obtain a range of age estimates for the most recent common ancestor of the genus Naso .
	manualset3
201054	2	417421	7	NULL	NULL	0	NULL	nuclear marker , ETS2	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	We used a genus-level phylogeny ( nuclear marker , ETS2 ) , which included several taxa from all other acanthurid genera , to obtain a range of age estimates for the most recent common ancestor of the genus Naso .
	manualset3
201057	3	417421	7	NULL	NULL	0	NULL	taxa	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We used a genus-level phylogeny ( nuclear marker , ETS2 ) , which included several taxa from all other acanthurid genera , to obtain a range of age estimates for the most recent common ancestor of the genus Naso .
	manualset3
201059	4	417421	7	NULL	NULL	0	NULL	acanthurid genera	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We used a genus-level phylogeny ( nuclear marker , ETS2 ) , which included several taxa from all other acanthurid genera , to obtain a range of age estimates for the most recent common ancestor of the genus Naso .
	manualset3
201060	5	417421	7	NULL	NULL	0	NULL	range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We used a genus-level phylogeny ( nuclear marker , ETS2 ) , which included several taxa from all other acanthurid genera , to obtain a range of age estimates for the most recent common ancestor of the genus Naso .
	manualset3
201061	6	417421	7	NULL	NULL	0	NULL	age estimates	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We used a genus-level phylogeny ( nuclear marker , ETS2 ) , which included several taxa from all other acanthurid genera , to obtain a range of age estimates for the most recent common ancestor of the genus Naso .
	manualset3
201062	7	417421	7	NULL	NULL	0	NULL	common ancestor	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We used a genus-level phylogeny ( nuclear marker , ETS2 ) , which included several taxa from all other acanthurid genera , to obtain a range of age estimates for the most recent common ancestor of the genus Naso .
	manualset3
201063	8	417421	7	NULL	NULL	0	NULL	genus Naso	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We used a genus-level phylogeny ( nuclear marker , ETS2 ) , which included several taxa from all other acanthurid genera , to obtain a range of age estimates for the most recent common ancestor of the genus Naso .
	manualset3
201064	1	417422	7	NULL	NULL	0	NULL	masking paradigm	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We used a masking paradigm to examine how visual sensitivity under these conditions compares with the perception of the direction of heading in real scenes ( i.e. , with dynamic natural images at high contrasts ) .
	manualset3
201065	2	417422	7	NULL	NULL	NULL	NULL	visual sensitivity	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We used a masking paradigm to examine how visual sensitivity under these conditions compares with the perception of the direction of heading in real scenes ( i.e. , with dynamic natural images at high contrasts ) .
	manualset3
201066	3	417422	7	NULL	NULL	0	NULL	conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We used a masking paradigm to examine how visual sensitivity under these conditions compares with the perception of the direction of heading in real scenes ( i.e. , with dynamic natural images at high contrasts ) .
	manualset3
201067	4	417422	7	NULL	NULL	0	NULL	perception	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We used a masking paradigm to examine how visual sensitivity under these conditions compares with the perception of the direction of heading in real scenes ( i.e. , with dynamic natural images at high contrasts ) .
	manualset3
201069	5	417422	7	NULL	NULL	0	NULL	direction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We used a masking paradigm to examine how visual sensitivity under these conditions compares with the perception of the direction of heading in real scenes ( i.e. , with dynamic natural images at high contrasts ) .
	manualset3
201072	6	417422	7	NULL	NULL	0	NULL	heading	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We used a masking paradigm to examine how visual sensitivity under these conditions compares with the perception of the direction of heading in real scenes ( i.e. , with dynamic natural images at high contrasts ) .
	manualset3
201073	7	417422	7	NULL	NULL	0	NULL	real scenes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We used a masking paradigm to examine how visual sensitivity under these conditions compares with the perception of the direction of heading in real scenes ( i.e. , with dynamic natural images at high contrasts ) .
	manualset3
201075	8	417422	7	NULL	NULL	0	NULL	dynamic natural images	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We used a masking paradigm to examine how visual sensitivity under these conditions compares with the perception of the direction of heading in real scenes ( i.e. , with dynamic natural images at high contrasts ) .
	manualset3
203097	9	417422	7	NULL	NULL	0	NULL	high contrasts	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We used a masking paradigm to examine how visual sensitivity under these conditions compares with the perception of the direction of heading in real scenes ( i.e. , with dynamic natural images at high contrasts ) .
	manualset3
201078	1	417423	7	NULL	NULL	0	NULL	stepwise approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We used a stepwise approach to identify , design , synthesize , and test new high atomic number particulate contrast agents that would be especially well suited for use with computed tomography ( CT ) .
	manualset3
201086	2	417423	7	NULL	NULL	0	NULL	high atomic number particulate contrast agents	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	We used a stepwise approach to identify , design , synthesize , and test new high atomic number particulate contrast agents that would be especially well suited for use with computed tomography ( CT ) .
	manualset3
201087	3	417423	7	NULL	NULL	0	NULL	computed tomography ( CT )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	We used a stepwise approach to identify , design , synthesize , and test new high atomic number particulate contrast agents that would be especially well suited for use with computed tomography ( CT ) .
	manualset3
201090	1	417424	7	NULL	NULL	0	NULL	immortalized , hypothalamic , clonal cell line , mHypoE-46	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We used an immortalized , hypothalamic , clonal cell line , mHypoE-46 , which exemplifies neuronal function and expresses the components of the insulin signaling pathway , to determine how hyperinsulinemia modifies neuronal function .
	manualset3
201091	2	417424	7	NULL	NULL	0	NULL	neuronal function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We used an immortalized , hypothalamic , clonal cell line , mHypoE-46 , which exemplifies neuronal function and expresses the components of the insulin signaling pathway , to determine how hyperinsulinemia modifies neuronal function .
	manualset3
201092	3	417424	7	NULL	NULL	0	NULL	 components	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We used an immortalized , hypothalamic , clonal cell line , mHypoE-46 , which exemplifies neuronal function and expresses the components of the insulin signaling pathway , to determine how hyperinsulinemia modifies neuronal function .
	manualset3
201093	4	417424	7	NULL	NULL	0	NULL	 insulin signaling pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We used an immortalized , hypothalamic , clonal cell line , mHypoE-46 , which exemplifies neuronal function and expresses the components of the insulin signaling pathway , to determine how hyperinsulinemia modifies neuronal function .
	manualset3
201094	5	417424	7	NULL	NULL	0	NULL	hyperinsulinemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We used an immortalized , hypothalamic , clonal cell line , mHypoE-46 , which exemplifies neuronal function and expresses the components of the insulin signaling pathway , to determine how hyperinsulinemia modifies neuronal function .
	manualset3
201096	6	417424	7	NULL	NULL	0	NULL	 neuronal function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We used an immortalized , hypothalamic , clonal cell line , mHypoE-46 , which exemplifies neuronal function and expresses the components of the insulin signaling pathway , to determine how hyperinsulinemia modifies neuronal function .
	manualset3
201099	1	417425	7	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	We used data from the Pediatric HIV/AIDS Cohort Study ( PHACS ) Surveillance Monitoring for ART Toxicities ( SMARTT ) study , a United States-based prospective cohort study of HIV-exposed but uninfected children , to assess temporal trends and maternal characteristics associated with the use of ARVs during pregnancy .
	manualset3
201101	2	417425	7	NULL	NULL	NULL	NULL	Pediatric HIV/AIDS Cohort Study ( PHACS )	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We used data from the Pediatric HIV/AIDS Cohort Study ( PHACS ) Surveillance Monitoring for ART Toxicities ( SMARTT ) study , a United States-based prospective cohort study of HIV-exposed but uninfected children , to assess temporal trends and maternal characteristics associated with the use of ARVs during pregnancy .
	manualset3
201102	3	417425	7	NULL	NULL	0	NULL	United States-based prospective cohort study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We used data from the Pediatric HIV/AIDS Cohort Study ( PHACS ) Surveillance Monitoring for ART Toxicities ( SMARTT ) study , a United States-based prospective cohort study of HIV-exposed but uninfected children , to assess temporal trends and maternal characteristics associated with the use of ARVs during pregnancy .
	manualset3
201105	4	417425	7	NULL	NULL	0	NULL	 uninfected children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We used data from the Pediatric HIV/AIDS Cohort Study ( PHACS ) Surveillance Monitoring for ART Toxicities ( SMARTT ) study , a United States-based prospective cohort study of HIV-exposed but uninfected children , to assess temporal trends and maternal characteristics associated with the use of ARVs during pregnancy .
	manualset3
201106	5	417425	7	NULL	NULL	NULL	NULL	 temporal trends	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We used data from the Pediatric HIV/AIDS Cohort Study ( PHACS ) Surveillance Monitoring for ART Toxicities ( SMARTT ) study , a United States-based prospective cohort study of HIV-exposed but uninfected children , to assess temporal trends and maternal characteristics associated with the use of ARVs during pregnancy .
	manualset3
201107	6	417425	7	NULL	NULL	0	NULL	maternal characteristics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We used data from the Pediatric HIV/AIDS Cohort Study ( PHACS ) Surveillance Monitoring for ART Toxicities ( SMARTT ) study , a United States-based prospective cohort study of HIV-exposed but uninfected children , to assess temporal trends and maternal characteristics associated with the use of ARVs during pregnancy .
	manualset3
201108	7	417425	7	NULL	NULL	0	NULL	ARVs 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	We used data from the Pediatric HIV/AIDS Cohort Study ( PHACS ) Surveillance Monitoring for ART Toxicities ( SMARTT ) study , a United States-based prospective cohort study of HIV-exposed but uninfected children , to assess temporal trends and maternal characteristics associated with the use of ARVs during pregnancy .
	manualset3
201109	8	417425	7	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We used data from the Pediatric HIV/AIDS Cohort Study ( PHACS ) Surveillance Monitoring for ART Toxicities ( SMARTT ) study , a United States-based prospective cohort study of HIV-exposed but uninfected children , to assess temporal trends and maternal characteristics associated with the use of ARVs during pregnancy .
	manualset3
201110	9	417425	7	NULL	NULL	0	NULL	 Surveillance Monitoring for ART Toxicities ( SMARTT ) study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We used data from the Pediatric HIV/AIDS Cohort Study ( PHACS ) Surveillance Monitoring for ART Toxicities ( SMARTT ) study , a United States-based prospective cohort study of HIV-exposed but uninfected children , to assess temporal trends and maternal characteristics associated with the use of ARVs during pregnancy .
	manualset3
201111	1	417426	7	NULL	NULL	0	NULL	microarrays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We used dedicated microarrays to compare gene expression among the duodenum of Hfe ( - / - ) mice , induced iron overload mice , and control mice .
	manualset3
201112	2	417426	7	NULL	NULL	0	NULL	 gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We used dedicated microarrays to compare gene expression among the duodenum of Hfe ( - / - ) mice , induced iron overload mice , and control mice .
	manualset3
201113	3	417426	7	NULL	NULL	0	NULL	duodenum 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We used dedicated microarrays to compare gene expression among the duodenum of Hfe ( - / - ) mice , induced iron overload mice , and control mice .
	manualset3
201114	4	417426	7	NULL	NULL	0	NULL	Hfe ( - / - ) mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We used dedicated microarrays to compare gene expression among the duodenum of Hfe ( - / - ) mice , induced iron overload mice , and control mice .
	manualset3
201115	5	417426	7	NULL	NULL	0	NULL	 induced iron overload mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We used dedicated microarrays to compare gene expression among the duodenum of Hfe ( - / - ) mice , induced iron overload mice , and control mice .
	manualset3
201116	6	417426	7	NULL	NULL	0	NULL	control mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We used dedicated microarrays to compare gene expression among the duodenum of Hfe ( - / - ) mice , induced iron overload mice , and control mice .
	manualset3
201117	1	417427	7	NULL	NULL	0	NULL	echocardiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	We used echocardiography and tissue Doppler imaging to investigate the effects on RV and LV function of 90 min of hypoxic breathing ( fraction of inspired O ( 2 ) of 0.12 ) compared with those of dobutamine to reproduce the same heart rate effects without change in pulmonary vascular tone in 25 healthy volunteers .
	manualset3
201118	2	417427	7	NULL	NULL	0	NULL	tissue Doppler imaging 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	We used echocardiography and tissue Doppler imaging to investigate the effects on RV and LV function of 90 min of hypoxic breathing ( fraction of inspired O ( 2 ) of 0.12 ) compared with those of dobutamine to reproduce the same heart rate effects without change in pulmonary vascular tone in 25 healthy volunteers .
	manualset3
201119	3	417427	7	NULL	NULL	0	NULL	effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We used echocardiography and tissue Doppler imaging to investigate the effects on RV and LV function of 90 min of hypoxic breathing ( fraction of inspired O ( 2 ) of 0.12 ) compared with those of dobutamine to reproduce the same heart rate effects without change in pulmonary vascular tone in 25 healthy volunteers .
	manualset3
201120	4	417427	7	NULL	NULL	0	NULL	RV function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We used echocardiography and tissue Doppler imaging to investigate the effects on RV and LV function of 90 min of hypoxic breathing ( fraction of inspired O ( 2 ) of 0.12 ) compared with those of dobutamine to reproduce the same heart rate effects without change in pulmonary vascular tone in 25 healthy volunteers .
	manualset3
201121	5	417427	7	NULL	NULL	0	NULL	LV function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We used echocardiography and tissue Doppler imaging to investigate the effects on RV and LV function of 90 min of hypoxic breathing ( fraction of inspired O ( 2 ) of 0.12 ) compared with those of dobutamine to reproduce the same heart rate effects without change in pulmonary vascular tone in 25 healthy volunteers .
	manualset3
201122	6	417427	7	NULL	NULL	0	NULL	90 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	We used echocardiography and tissue Doppler imaging to investigate the effects on RV and LV function of 90 min of hypoxic breathing ( fraction of inspired O ( 2 ) of 0.12 ) compared with those of dobutamine to reproduce the same heart rate effects without change in pulmonary vascular tone in 25 healthy volunteers .
	manualset3
201123	7	417427	7	NULL	NULL	0	NULL	 hypoxic breathing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We used echocardiography and tissue Doppler imaging to investigate the effects on RV and LV function of 90 min of hypoxic breathing ( fraction of inspired O ( 2 ) of 0.12 ) compared with those of dobutamine to reproduce the same heart rate effects without change in pulmonary vascular tone in 25 healthy volunteers .
	manualset3
201124	8	417427	7	NULL	NULL	0	NULL	fraction	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We used echocardiography and tissue Doppler imaging to investigate the effects on RV and LV function of 90 min of hypoxic breathing ( fraction of inspired O ( 2 ) of 0.12 ) compared with those of dobutamine to reproduce the same heart rate effects without change in pulmonary vascular tone in 25 healthy volunteers .
	manualset3
201125	9	417427	7	NULL	NULL	0	NULL	inspired O ( 2 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We used echocardiography and tissue Doppler imaging to investigate the effects on RV and LV function of 90 min of hypoxic breathing ( fraction of inspired O ( 2 ) of 0.12 ) compared with those of dobutamine to reproduce the same heart rate effects without change in pulmonary vascular tone in 25 healthy volunteers .
	manualset3
201126	10	417427	7	NULL	NULL	0	NULL	 0.12	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	We used echocardiography and tissue Doppler imaging to investigate the effects on RV and LV function of 90 min of hypoxic breathing ( fraction of inspired O ( 2 ) of 0.12 ) compared with those of dobutamine to reproduce the same heart rate effects without change in pulmonary vascular tone in 25 healthy volunteers .
	manualset3
201127	11	417427	7	NULL	NULL	0	NULL	dobutamine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	We used echocardiography and tissue Doppler imaging to investigate the effects on RV and LV function of 90 min of hypoxic breathing ( fraction of inspired O ( 2 ) of 0.12 ) compared with those of dobutamine to reproduce the same heart rate effects without change in pulmonary vascular tone in 25 healthy volunteers .
	manualset3
201128	12	417427	7	NULL	NULL	0	NULL	heart rate effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We used echocardiography and tissue Doppler imaging to investigate the effects on RV and LV function of 90 min of hypoxic breathing ( fraction of inspired O ( 2 ) of 0.12 ) compared with those of dobutamine to reproduce the same heart rate effects without change in pulmonary vascular tone in 25 healthy volunteers .
	manualset3
201129	13	417427	7	NULL	NULL	0	NULL	change 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We used echocardiography and tissue Doppler imaging to investigate the effects on RV and LV function of 90 min of hypoxic breathing ( fraction of inspired O ( 2 ) of 0.12 ) compared with those of dobutamine to reproduce the same heart rate effects without change in pulmonary vascular tone in 25 healthy volunteers .
	manualset3
201130	14	417427	7	NULL	NULL	0	NULL	pulmonary vascular tone	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We used echocardiography and tissue Doppler imaging to investigate the effects on RV and LV function of 90 min of hypoxic breathing ( fraction of inspired O ( 2 ) of 0.12 ) compared with those of dobutamine to reproduce the same heart rate effects without change in pulmonary vascular tone in 25 healthy volunteers .
	manualset3
201131	15	417427	7	NULL	NULL	0	NULL	25 healthy volunteers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We used echocardiography and tissue Doppler imaging to investigate the effects on RV and LV function of 90 min of hypoxic breathing ( fraction of inspired O ( 2 ) of 0.12 ) compared with those of dobutamine to reproduce the same heart rate effects without change in pulmonary vascular tone in 25 healthy volunteers .
	manualset3
201132	1	417428	7	NULL	NULL	0	NULL	infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All infants had neurologic manifestations of asphyxia and required assisted ventilation .
	manualset3
201133	2	417428	7	NULL	NULL	0	NULL	neurologic manifestations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All infants had neurologic manifestations of asphyxia and required assisted ventilation .
	manualset3
201134	3	417428	7	NULL	NULL	0	NULL	asphyxia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All infants had neurologic manifestations of asphyxia and required assisted ventilation .
	manualset3
201135	4	417428	7	NULL	NULL	0	NULL	assisted ventilation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All infants had neurologic manifestations of asphyxia and required assisted ventilation .
	manualset3
201136	1	417429	7	NULL	NULL	0	NULL	 immunological techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We used immunological techniques to compare the serum corticosteroid-binding globulins ( CBG ) and testosterone-estradiol-binding globulins ( TeBG ) of Old World primates ( man , chimpanzee , cynomologus , and rhesus ) , New World monkeys ( squirrel and owl ) , and prosimians ( galago and lemur ) .
	manualset3
201137	2	417429	7	NULL	NULL	0	NULL	 serum corticosteroid-binding globulins ( CBG )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We used immunological techniques to compare the serum corticosteroid-binding globulins ( CBG ) and testosterone-estradiol-binding globulins ( TeBG ) of Old World primates ( man , chimpanzee , cynomologus , and rhesus ) , New World monkeys ( squirrel and owl ) , and prosimians ( galago and lemur ) .
	manualset3
201138	3	417429	7	NULL	NULL	0	NULL	testosterone-estradiol-binding globulins ( TeBG )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We used immunological techniques to compare the serum corticosteroid-binding globulins ( CBG ) and testosterone-estradiol-binding globulins ( TeBG ) of Old World primates ( man , chimpanzee , cynomologus , and rhesus ) , New World monkeys ( squirrel and owl ) , and prosimians ( galago and lemur ) .
	manualset3
201139	4	417429	7	NULL	NULL	0	NULL	Old World primates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We used immunological techniques to compare the serum corticosteroid-binding globulins ( CBG ) and testosterone-estradiol-binding globulins ( TeBG ) of Old World primates ( man , chimpanzee , cynomologus , and rhesus ) , New World monkeys ( squirrel and owl ) , and prosimians ( galago and lemur ) .
	manualset3
201140	5	417429	7	NULL	NULL	0	NULL	man	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We used immunological techniques to compare the serum corticosteroid-binding globulins ( CBG ) and testosterone-estradiol-binding globulins ( TeBG ) of Old World primates ( man , chimpanzee , cynomologus , and rhesus ) , New World monkeys ( squirrel and owl ) , and prosimians ( galago and lemur ) .
	manualset3
201141	6	417429	7	NULL	NULL	0	NULL	chimpanzee	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We used immunological techniques to compare the serum corticosteroid-binding globulins ( CBG ) and testosterone-estradiol-binding globulins ( TeBG ) of Old World primates ( man , chimpanzee , cynomologus , and rhesus ) , New World monkeys ( squirrel and owl ) , and prosimians ( galago and lemur ) .
	manualset3
201142	7	417429	7	NULL	NULL	0	NULL	cynomologus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We used immunological techniques to compare the serum corticosteroid-binding globulins ( CBG ) and testosterone-estradiol-binding globulins ( TeBG ) of Old World primates ( man , chimpanzee , cynomologus , and rhesus ) , New World monkeys ( squirrel and owl ) , and prosimians ( galago and lemur ) .
	manualset3
201143	8	417429	7	NULL	NULL	0	NULL	rhesus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We used immunological techniques to compare the serum corticosteroid-binding globulins ( CBG ) and testosterone-estradiol-binding globulins ( TeBG ) of Old World primates ( man , chimpanzee , cynomologus , and rhesus ) , New World monkeys ( squirrel and owl ) , and prosimians ( galago and lemur ) .
	manualset3
201144	9	417429	7	NULL	NULL	0	NULL	New World monkeys	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We used immunological techniques to compare the serum corticosteroid-binding globulins ( CBG ) and testosterone-estradiol-binding globulins ( TeBG ) of Old World primates ( man , chimpanzee , cynomologus , and rhesus ) , New World monkeys ( squirrel and owl ) , and prosimians ( galago and lemur ) .
	manualset3
201145	10	417429	7	NULL	NULL	0	NULL	squirrel	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We used immunological techniques to compare the serum corticosteroid-binding globulins ( CBG ) and testosterone-estradiol-binding globulins ( TeBG ) of Old World primates ( man , chimpanzee , cynomologus , and rhesus ) , New World monkeys ( squirrel and owl ) , and prosimians ( galago and lemur ) .
	manualset3
201146	11	417429	7	NULL	NULL	0	NULL	owl 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We used immunological techniques to compare the serum corticosteroid-binding globulins ( CBG ) and testosterone-estradiol-binding globulins ( TeBG ) of Old World primates ( man , chimpanzee , cynomologus , and rhesus ) , New World monkeys ( squirrel and owl ) , and prosimians ( galago and lemur ) .
	manualset3
201147	12	417429	7	NULL	NULL	0	NULL	prosimians	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We used immunological techniques to compare the serum corticosteroid-binding globulins ( CBG ) and testosterone-estradiol-binding globulins ( TeBG ) of Old World primates ( man , chimpanzee , cynomologus , and rhesus ) , New World monkeys ( squirrel and owl ) , and prosimians ( galago and lemur ) .
	manualset3
201149	13	417429	7	NULL	NULL	0	NULL	galago	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We used immunological techniques to compare the serum corticosteroid-binding globulins ( CBG ) and testosterone-estradiol-binding globulins ( TeBG ) of Old World primates ( man , chimpanzee , cynomologus , and rhesus ) , New World monkeys ( squirrel and owl ) , and prosimians ( galago and lemur ) .
	manualset3
201152	14	417429	7	NULL	NULL	0	NULL	lemur	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We used immunological techniques to compare the serum corticosteroid-binding globulins ( CBG ) and testosterone-estradiol-binding globulins ( TeBG ) of Old World primates ( man , chimpanzee , cynomologus , and rhesus ) , New World monkeys ( squirrel and owl ) , and prosimians ( galago and lemur ) .
	manualset3
201157	1	417430	7	NULL	NULL	0	NULL	linear and multinomial models 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We used linear and multinomial models to partition the variation in BMI ( in kg/m ( 2 ) ) , underweight ( BMI & lt ; 18.5 kg/m ( 2 ) ) and overweight ( BMI 25.0 kg/m ( 2 ) ) at the level of neighborhoods and countries .
	manualset3
201160	2	417430	7	NULL	NULL	0	NULL	 variation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We used linear and multinomial models to partition the variation in BMI ( in kg/m ( 2 ) ) , underweight ( BMI & lt ; 18.5 kg/m ( 2 ) ) and overweight ( BMI 25.0 kg/m ( 2 ) ) at the level of neighborhoods and countries .
	manualset3
201162	3	417430	7	NULL	NULL	0	NULL	BMI	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We used linear and multinomial models to partition the variation in BMI ( in kg/m ( 2 ) ) , underweight ( BMI & lt ; 18.5 kg/m ( 2 ) ) and overweight ( BMI 25.0 kg/m ( 2 ) ) at the level of neighborhoods and countries .
	manualset3
201163	4	417430	7	NULL	NULL	0	NULL	kg/m ( 2 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We used linear and multinomial models to partition the variation in BMI ( in kg/m ( 2 ) ) , underweight ( BMI & lt ; 18.5 kg/m ( 2 ) ) and overweight ( BMI 25.0 kg/m ( 2 ) ) at the level of neighborhoods and countries .
	manualset3
201164	5	417430	7	NULL	NULL	0	NULL	underweight	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We used linear and multinomial models to partition the variation in BMI ( in kg/m ( 2 ) ) , underweight ( BMI & lt ; 18.5 kg/m ( 2 ) ) and overweight ( BMI 25.0 kg/m ( 2 ) ) at the level of neighborhoods and countries .
	manualset3
201167	6	417430	7	NULL	NULL	0	NULL	BMI	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We used linear and multinomial models to partition the variation in BMI ( in kg/m ( 2 ) ) , underweight ( BMI & lt ; 18.5 kg/m ( 2 ) ) and overweight ( BMI 25.0 kg/m ( 2 ) ) at the level of neighborhoods and countries .
	manualset3
201168	7	417430	7	NULL	NULL	0	NULL	 lt	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We used linear and multinomial models to partition the variation in BMI ( in kg/m ( 2 ) ) , underweight ( BMI & lt ; 18.5 kg/m ( 2 ) ) and overweight ( BMI 25.0 kg/m ( 2 ) ) at the level of neighborhoods and countries .
	manualset3
201171	8	417430	7	NULL	NULL	0	NULL	18.5 kg/m ( 2 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	We used linear and multinomial models to partition the variation in BMI ( in kg/m ( 2 ) ) , underweight ( BMI & lt ; 18.5 kg/m ( 2 ) ) and overweight ( BMI 25.0 kg/m ( 2 ) ) at the level of neighborhoods and countries .
	manualset3
201172	9	417430	7	NULL	NULL	0	NULL	overweight	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We used linear and multinomial models to partition the variation in BMI ( in kg/m ( 2 ) ) , underweight ( BMI & lt ; 18.5 kg/m ( 2 ) ) and overweight ( BMI 25.0 kg/m ( 2 ) ) at the level of neighborhoods and countries .
	manualset3
201173	10	417430	7	NULL	NULL	0	NULL	BMI	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We used linear and multinomial models to partition the variation in BMI ( in kg/m ( 2 ) ) , underweight ( BMI & lt ; 18.5 kg/m ( 2 ) ) and overweight ( BMI 25.0 kg/m ( 2 ) ) at the level of neighborhoods and countries .
	manualset3
201174	11	417430	7	NULL	NULL	0	NULL	25.0 kg/m ( 2 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	We used linear and multinomial models to partition the variation in BMI ( in kg/m ( 2 ) ) , underweight ( BMI & lt ; 18.5 kg/m ( 2 ) ) and overweight ( BMI 25.0 kg/m ( 2 ) ) at the level of neighborhoods and countries .
	manualset3
201175	12	417430	7	NULL	NULL	0	NULL	level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We used linear and multinomial models to partition the variation in BMI ( in kg/m ( 2 ) ) , underweight ( BMI & lt ; 18.5 kg/m ( 2 ) ) and overweight ( BMI 25.0 kg/m ( 2 ) ) at the level of neighborhoods and countries .
	manualset3
201176	13	417430	7	NULL	NULL	0	NULL	countries	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	We used linear and multinomial models to partition the variation in BMI ( in kg/m ( 2 ) ) , underweight ( BMI & lt ; 18.5 kg/m ( 2 ) ) and overweight ( BMI 25.0 kg/m ( 2 ) ) at the level of neighborhoods and countries .
	manualset3
201177	14	417430	7	NULL	NULL	0	NULL	neighborhoods 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We used linear and multinomial models to partition the variation in BMI ( in kg/m ( 2 ) ) , underweight ( BMI & lt ; 18.5 kg/m ( 2 ) ) and overweight ( BMI 25.0 kg/m ( 2 ) ) at the level of neighborhoods and countries .
	manualset3
201745	1	417431	7	NULL	NULL	0	NULL	microarrays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We used microarrays and analysis of soil physicochemical variables to investigate the methane-oxidizing communities of several Australian natural woodland soils affected to varying degrees by dryland salinity .
	manualset3
201746	2	417431	7	NULL	NULL	0	NULL	analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We used microarrays and analysis of soil physicochemical variables to investigate the methane-oxidizing communities of several Australian natural woodland soils affected to varying degrees by dryland salinity .
	manualset3
201747	3	417431	7	NULL	NULL	0	NULL	soil physicochemical variables	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We used microarrays and analysis of soil physicochemical variables to investigate the methane-oxidizing communities of several Australian natural woodland soils affected to varying degrees by dryland salinity .
	manualset3
201748	4	417431	7	NULL	NULL	0	NULL	methane-oxidizing communities 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We used microarrays and analysis of soil physicochemical variables to investigate the methane-oxidizing communities of several Australian natural woodland soils affected to varying degrees by dryland salinity .
	manualset3
201749	5	417431	7	NULL	NULL	0	NULL	Australian natural woodland soils	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We used microarrays and analysis of soil physicochemical variables to investigate the methane-oxidizing communities of several Australian natural woodland soils affected to varying degrees by dryland salinity .
	manualset3
201750	6	417431	7	NULL	NULL	0	NULL	 varying degrees 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We used microarrays and analysis of soil physicochemical variables to investigate the methane-oxidizing communities of several Australian natural woodland soils affected to varying degrees by dryland salinity .
	manualset3
201751	7	417431	7	NULL	NULL	0	NULL	 dryland salinity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We used microarrays and analysis of soil physicochemical variables to investigate the methane-oxidizing communities of several Australian natural woodland soils affected to varying degrees by dryland salinity .
	manualset3
201752	1	417432	7	NULL	NULL	0	NULL	replicate lines 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We used replicate lines of yellow dung flies Scathophaga stercoraria ( L. ) with different PO levels to investigate whether PO levels affect resistance against parasitic mites and entomopathogenic fungi .
	manualset3
201753	2	417432	7	NULL	NULL	0	NULL	yellow dung flies	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We used replicate lines of yellow dung flies Scathophaga stercoraria ( L. ) with different PO levels to investigate whether PO levels affect resistance against parasitic mites and entomopathogenic fungi .
	manualset3
201754	3	417432	7	NULL	NULL	0	NULL	Scathophaga stercoraria ( L. ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We used replicate lines of yellow dung flies Scathophaga stercoraria ( L. ) with different PO levels to investigate whether PO levels affect resistance against parasitic mites and entomopathogenic fungi .
	manualset3
201755	4	417432	7	NULL	NULL	0	NULL	 different PO levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We used replicate lines of yellow dung flies Scathophaga stercoraria ( L. ) with different PO levels to investigate whether PO levels affect resistance against parasitic mites and entomopathogenic fungi .
	manualset3
201756	5	417432	7	NULL	NULL	0	NULL	PO levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We used replicate lines of yellow dung flies Scathophaga stercoraria ( L. ) with different PO levels to investigate whether PO levels affect resistance against parasitic mites and entomopathogenic fungi .
	manualset3
201757	6	417432	7	NULL	NULL	0	NULL	parasitic mites	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We used replicate lines of yellow dung flies Scathophaga stercoraria ( L. ) with different PO levels to investigate whether PO levels affect resistance against parasitic mites and entomopathogenic fungi .
	manualset3
201758	7	417432	7	NULL	NULL	0	NULL	entomopathogenic fungi	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We used replicate lines of yellow dung flies Scathophaga stercoraria ( L. ) with different PO levels to investigate whether PO levels affect resistance against parasitic mites and entomopathogenic fungi .
	manualset3
204389	8	417432	7	NULL	NULL	0	NULL	resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We used replicate lines of yellow dung flies Scathophaga stercoraria ( L. ) with different PO levels to investigate whether PO levels affect resistance against parasitic mites and entomopathogenic fungi .
	manualset3
201759	1	417433	7	NULL	NULL	0	NULL	coexpression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We used the coexpression of biotin ligase and acceptor protein to label the biotin-domain peptide in vitro with ( 3H ) biotin , which greatly facilitated development of a purification procedure .
	manualset3
201760	2	417433	7	NULL	NULL	0	NULL	 biotin ligase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We used the coexpression of biotin ligase and acceptor protein to label the biotin-domain peptide in vitro with ( 3H ) biotin , which greatly facilitated development of a purification procedure .
	manualset3
201761	3	417433	7	NULL	NULL	0	NULL	acceptor protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We used the coexpression of biotin ligase and acceptor protein to label the biotin-domain peptide in vitro with ( 3H ) biotin , which greatly facilitated development of a purification procedure .
	manualset3
201762	4	417433	7	NULL	NULL	0	NULL	biotin-domain peptide	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	We used the coexpression of biotin ligase and acceptor protein to label the biotin-domain peptide in vitro with ( 3H ) biotin , which greatly facilitated development of a purification procedure .
	manualset3
201763	5	417433	7	NULL	NULL	0	NULL	( 3H ) biotin 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We used the coexpression of biotin ligase and acceptor protein to label the biotin-domain peptide in vitro with ( 3H ) biotin , which greatly facilitated development of a purification procedure .
	manualset3
201764	6	417433	7	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We used the coexpression of biotin ligase and acceptor protein to label the biotin-domain peptide in vitro with ( 3H ) biotin , which greatly facilitated development of a purification procedure .
	manualset3
201765	7	417433	7	NULL	NULL	0	NULL	purification procedure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We used the coexpression of biotin ligase and acceptor protein to label the biotin-domain peptide in vitro with ( 3H ) biotin , which greatly facilitated development of a purification procedure .
	manualset3
201766	1	417434	7	NULL	NULL	0	NULL	hypomorphic Egfr ( wa2 ) allele	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	We used the hypomorphic Egfr ( wa2 ) allele to genetically examine the impact of impaired epidermal growth factor receptor ( Egfr ) signaling on the Apc ( Min ) mouse model of familial adenomatous polyposis .
	manualset3
201767	2	417434	7	NULL	NULL	NULL	NULL	 impact	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We used the hypomorphic Egfr ( wa2 ) allele to genetically examine the impact of impaired epidermal growth factor receptor ( Egfr ) signaling on the Apc ( Min ) mouse model of familial adenomatous polyposis .
	manualset3
201768	3	417434	7	NULL	NULL	0	NULL	impaired epidermal growth factor receptor ( Egfr ) signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We used the hypomorphic Egfr ( wa2 ) allele to genetically examine the impact of impaired epidermal growth factor receptor ( Egfr ) signaling on the Apc ( Min ) mouse model of familial adenomatous polyposis .
	manualset3
201769	4	417434	7	NULL	NULL	0	NULL	Apc ( Min ) mouse model 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We used the hypomorphic Egfr ( wa2 ) allele to genetically examine the impact of impaired epidermal growth factor receptor ( Egfr ) signaling on the Apc ( Min ) mouse model of familial adenomatous polyposis .
	manualset3
201770	5	417434	7	NULL	NULL	0	NULL	familial adenomatous polyposis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We used the hypomorphic Egfr ( wa2 ) allele to genetically examine the impact of impaired epidermal growth factor receptor ( Egfr ) signaling on the Apc ( Min ) mouse model of familial adenomatous polyposis .
	manualset3
201771	1	417435	7	NULL	NULL	0	NULL	 three different types	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We used three different types of artificial gene networks ( AGNs ) with distinct topologies : topologies random ( RND ) , scale-free ( SF ) , and small-world ( SW ) , to investigate their robustness and identifiability .
	manualset3
201772	2	417435	7	NULL	NULL	0	NULL	 artificial gene networks ( AGNs )	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We used three different types of artificial gene networks ( AGNs ) with distinct topologies : topologies random ( RND ) , scale-free ( SF ) , and small-world ( SW ) , to investigate their robustness and identifiability .
	manualset3
201773	3	417435	7	NULL	NULL	0	NULL	topologies	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We used three different types of artificial gene networks ( AGNs ) with distinct topologies : topologies random ( RND ) , scale-free ( SF ) , and small-world ( SW ) , to investigate their robustness and identifiability .
	manualset3
201774	4	417435	7	NULL	NULL	0	NULL	topologies random ( RND ) 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We used three different types of artificial gene networks ( AGNs ) with distinct topologies : topologies random ( RND ) , scale-free ( SF ) , and small-world ( SW ) , to investigate their robustness and identifiability .
	manualset3
201775	5	417435	7	NULL	NULL	0	NULL	scale-free ( SF )	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We used three different types of artificial gene networks ( AGNs ) with distinct topologies : topologies random ( RND ) , scale-free ( SF ) , and small-world ( SW ) , to investigate their robustness and identifiability .
	manualset3
201776	6	417435	7	NULL	NULL	0	NULL	small-world ( SW )	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We used three different types of artificial gene networks ( AGNs ) with distinct topologies : topologies random ( RND ) , scale-free ( SF ) , and small-world ( SW ) , to investigate their robustness and identifiability .
	manualset3
201777	7	417435	7	NULL	NULL	0	NULL	identifiability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We used three different types of artificial gene networks ( AGNs ) with distinct topologies : topologies random ( RND ) , scale-free ( SF ) , and small-world ( SW ) , to investigate their robustness and identifiability .
	manualset3
205461	8	417435	7	NULL	NULL	0	NULL	robustness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We used three different types of artificial gene networks ( AGNs ) with distinct topologies : topologies random ( RND ) , scale-free ( SF ) , and small-world ( SW ) , to investigate their robustness and identifiability .
	manualset3
201778	1	417436	7	NULL	NULL	0	NULL	three genetically differentiated Drosophila subobscura populations 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We used three genetically differentiated Drosophila subobscura populations according to inversion polymorphism analysis and measured the variability of sternopleural bristle number and change in FA across generations P , F1 , and F2 between intra - and interpopulation hybrids of D. subobscura .
	manualset3
201779	2	417436	7	NULL	NULL	0	NULL	inversion polymorphism analysis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We used three genetically differentiated Drosophila subobscura populations according to inversion polymorphism analysis and measured the variability of sternopleural bristle number and change in FA across generations P , F1 , and F2 between intra - and interpopulation hybrids of D. subobscura .
	manualset3
201780	3	417436	7	NULL	NULL	0	NULL	variability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We used three genetically differentiated Drosophila subobscura populations according to inversion polymorphism analysis and measured the variability of sternopleural bristle number and change in FA across generations P , F1 , and F2 between intra - and interpopulation hybrids of D. subobscura .
	manualset3
201781	4	417436	7	NULL	NULL	0	NULL	sternopleural bristle number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We used three genetically differentiated Drosophila subobscura populations according to inversion polymorphism analysis and measured the variability of sternopleural bristle number and change in FA across generations P , F1 , and F2 between intra - and interpopulation hybrids of D. subobscura .
	manualset3
201782	5	417436	7	NULL	NULL	0	NULL	change	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We used three genetically differentiated Drosophila subobscura populations according to inversion polymorphism analysis and measured the variability of sternopleural bristle number and change in FA across generations P , F1 , and F2 between intra - and interpopulation hybrids of D. subobscura .
	manualset3
201783	6	417436	7	NULL	NULL	0	NULL	FA	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We used three genetically differentiated Drosophila subobscura populations according to inversion polymorphism analysis and measured the variability of sternopleural bristle number and change in FA across generations P , F1 , and F2 between intra - and interpopulation hybrids of D. subobscura .
	manualset3
201784	7	417436	7	NULL	NULL	0	NULL	generations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We used three genetically differentiated Drosophila subobscura populations according to inversion polymorphism analysis and measured the variability of sternopleural bristle number and change in FA across generations P , F1 , and F2 between intra - and interpopulation hybrids of D. subobscura .
	manualset3
201785	8	417436	7	NULL	NULL	0	NULL	P 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We used three genetically differentiated Drosophila subobscura populations according to inversion polymorphism analysis and measured the variability of sternopleural bristle number and change in FA across generations P , F1 , and F2 between intra - and interpopulation hybrids of D. subobscura .
	manualset3
201786	9	417436	7	NULL	NULL	NULL	NULL	F1	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We used three genetically differentiated Drosophila subobscura populations according to inversion polymorphism analysis and measured the variability of sternopleural bristle number and change in FA across generations P , F1 , and F2 between intra - and interpopulation hybrids of D. subobscura .
	manualset3
201787	10	417436	7	NULL	NULL	0	NULL	F2	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We used three genetically differentiated Drosophila subobscura populations according to inversion polymorphism analysis and measured the variability of sternopleural bristle number and change in FA across generations P , F1 , and F2 between intra - and interpopulation hybrids of D. subobscura .
	manualset3
201788	11	417436	7	NULL	NULL	NULL	NULL	intra - population hybrids	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We used three genetically differentiated Drosophila subobscura populations according to inversion polymorphism analysis and measured the variability of sternopleural bristle number and change in FA across generations P , F1 , and F2 between intra - and interpopulation hybrids of D. subobscura .
	manualset3
201789	12	417436	7	NULL	NULL	NULL	NULL	interpopulation hybrids	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We used three genetically differentiated Drosophila subobscura populations according to inversion polymorphism analysis and measured the variability of sternopleural bristle number and change in FA across generations P , F1 , and F2 between intra - and interpopulation hybrids of D. subobscura .
	manualset3
201790	13	417436	7	NULL	NULL	0	NULL	 D. subobscura	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We used three genetically differentiated Drosophila subobscura populations according to inversion polymorphism analysis and measured the variability of sternopleural bristle number and change in FA across generations P , F1 , and F2 between intra - and interpopulation hybrids of D. subobscura .
	manualset3
201850	1	417437	7	NULL	NULL	NULL	NULL	two culture matrix systems	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We used two culture matrix systems ( collagen sandwich and Matrigel ) to examine the responsiveness of albumin secretory function in cultured rat hepatocytes under various seeding conditions .
	manualset3
201851	2	417437	7	NULL	NULL	NULL	NULL	collagen sandwich	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We used two culture matrix systems ( collagen sandwich and Matrigel ) to examine the responsiveness of albumin secretory function in cultured rat hepatocytes under various seeding conditions .
	manualset3
201852	3	417437	7	NULL	NULL	NULL	NULL	 Matrigel	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We used two culture matrix systems ( collagen sandwich and Matrigel ) to examine the responsiveness of albumin secretory function in cultured rat hepatocytes under various seeding conditions .
	manualset3
201853	4	417437	7	NULL	NULL	0	NULL	responsiveness 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We used two culture matrix systems ( collagen sandwich and Matrigel ) to examine the responsiveness of albumin secretory function in cultured rat hepatocytes under various seeding conditions .
	manualset3
201854	5	417437	7	NULL	NULL	0	NULL	albumin secretory function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We used two culture matrix systems ( collagen sandwich and Matrigel ) to examine the responsiveness of albumin secretory function in cultured rat hepatocytes under various seeding conditions .
	manualset3
201855	6	417437	7	NULL	NULL	0	NULL	cultured rat hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We used two culture matrix systems ( collagen sandwich and Matrigel ) to examine the responsiveness of albumin secretory function in cultured rat hepatocytes under various seeding conditions .
	manualset3
201856	7	417437	7	NULL	NULL	0	NULL	seeding conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We used two culture matrix systems ( collagen sandwich and Matrigel ) to examine the responsiveness of albumin secretory function in cultured rat hepatocytes under various seeding conditions .
	manualset3
201857	1	417438	7	NULL	NULL	0	NULL	 cannabinoid receptor agonists	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We verified that neither the cannabinoid receptor agonists ( tetrahydrocannabinol ( 1-10 micromol/l ) , anandamide ( 0.1-10 micromol/l ) and CP 55 , 940 ( 5 nmol/l to 1 micromol/l ) ) , nor the specific CB1 and CB2 antagonists ( AM251 ( 10-500 nmol/l ) and AM630 ( 50 nmol/l to 1 micromol/l ) , respectively ) had a significant effect upon 3H-2-deoxy-D-glucose uptake by Caco-2 cells .
	manualset3
201858	2	417438	7	NULL	NULL	0	NULL	tetrahydrocannabinol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We verified that neither the cannabinoid receptor agonists ( tetrahydrocannabinol ( 1-10 micromol/l ) , anandamide ( 0.1-10 micromol/l ) and CP 55 , 940 ( 5 nmol/l to 1 micromol/l ) ) , nor the specific CB1 and CB2 antagonists ( AM251 ( 10-500 nmol/l ) and AM630 ( 50 nmol/l to 1 micromol/l ) , respectively ) had a significant effect upon 3H-2-deoxy-D-glucose uptake by Caco-2 cells .
	manualset3
201859	3	417438	7	NULL	NULL	0	NULL	1-10 micromol/l	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	We verified that neither the cannabinoid receptor agonists ( tetrahydrocannabinol ( 1-10 micromol/l ) , anandamide ( 0.1-10 micromol/l ) and CP 55 , 940 ( 5 nmol/l to 1 micromol/l ) ) , nor the specific CB1 and CB2 antagonists ( AM251 ( 10-500 nmol/l ) and AM630 ( 50 nmol/l to 1 micromol/l ) , respectively ) had a significant effect upon 3H-2-deoxy-D-glucose uptake by Caco-2 cells .
	manualset3
201860	4	417438	7	NULL	NULL	0	NULL	anandamide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We verified that neither the cannabinoid receptor agonists ( tetrahydrocannabinol ( 1-10 micromol/l ) , anandamide ( 0.1-10 micromol/l ) and CP 55 , 940 ( 5 nmol/l to 1 micromol/l ) ) , nor the specific CB1 and CB2 antagonists ( AM251 ( 10-500 nmol/l ) and AM630 ( 50 nmol/l to 1 micromol/l ) , respectively ) had a significant effect upon 3H-2-deoxy-D-glucose uptake by Caco-2 cells .
	manualset3
201861	5	417438	7	NULL	NULL	0	NULL	0.1-10 micromol/l	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	We verified that neither the cannabinoid receptor agonists ( tetrahydrocannabinol ( 1-10 micromol/l ) , anandamide ( 0.1-10 micromol/l ) and CP 55 , 940 ( 5 nmol/l to 1 micromol/l ) ) , nor the specific CB1 and CB2 antagonists ( AM251 ( 10-500 nmol/l ) and AM630 ( 50 nmol/l to 1 micromol/l ) , respectively ) had a significant effect upon 3H-2-deoxy-D-glucose uptake by Caco-2 cells .
	manualset3
201862	6	417438	7	NULL	NULL	0	NULL	CP 55 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We verified that neither the cannabinoid receptor agonists ( tetrahydrocannabinol ( 1-10 micromol/l ) , anandamide ( 0.1-10 micromol/l ) and CP 55 , 940 ( 5 nmol/l to 1 micromol/l ) ) , nor the specific CB1 and CB2 antagonists ( AM251 ( 10-500 nmol/l ) and AM630 ( 50 nmol/l to 1 micromol/l ) , respectively ) had a significant effect upon 3H-2-deoxy-D-glucose uptake by Caco-2 cells .
	manualset3
201863	7	417438	7	NULL	NULL	0	NULL	CP 940	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We verified that neither the cannabinoid receptor agonists ( tetrahydrocannabinol ( 1-10 micromol/l ) , anandamide ( 0.1-10 micromol/l ) and CP 55 , 940 ( 5 nmol/l to 1 micromol/l ) ) , nor the specific CB1 and CB2 antagonists ( AM251 ( 10-500 nmol/l ) and AM630 ( 50 nmol/l to 1 micromol/l ) , respectively ) had a significant effect upon 3H-2-deoxy-D-glucose uptake by Caco-2 cells .
	manualset3
201864	8	417438	7	NULL	NULL	0	NULL	5 nmol/l	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	We verified that neither the cannabinoid receptor agonists ( tetrahydrocannabinol ( 1-10 micromol/l ) , anandamide ( 0.1-10 micromol/l ) and CP 55 , 940 ( 5 nmol/l to 1 micromol/l ) ) , nor the specific CB1 and CB2 antagonists ( AM251 ( 10-500 nmol/l ) and AM630 ( 50 nmol/l to 1 micromol/l ) , respectively ) had a significant effect upon 3H-2-deoxy-D-glucose uptake by Caco-2 cells .
	manualset3
201865	9	417438	7	NULL	NULL	0	NULL	1 micromol/l 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	We verified that neither the cannabinoid receptor agonists ( tetrahydrocannabinol ( 1-10 micromol/l ) , anandamide ( 0.1-10 micromol/l ) and CP 55 , 940 ( 5 nmol/l to 1 micromol/l ) ) , nor the specific CB1 and CB2 antagonists ( AM251 ( 10-500 nmol/l ) and AM630 ( 50 nmol/l to 1 micromol/l ) , respectively ) had a significant effect upon 3H-2-deoxy-D-glucose uptake by Caco-2 cells .
	manualset3
201866	10	417438	7	NULL	NULL	0	NULL	specific CB1 antagonists	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We verified that neither the cannabinoid receptor agonists ( tetrahydrocannabinol ( 1-10 micromol/l ) , anandamide ( 0.1-10 micromol/l ) and CP 55 , 940 ( 5 nmol/l to 1 micromol/l ) ) , nor the specific CB1 and CB2 antagonists ( AM251 ( 10-500 nmol/l ) and AM630 ( 50 nmol/l to 1 micromol/l ) , respectively ) had a significant effect upon 3H-2-deoxy-D-glucose uptake by Caco-2 cells .
	manualset3
201867	11	417438	7	NULL	NULL	0	NULL	specific CB2 antagonists	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We verified that neither the cannabinoid receptor agonists ( tetrahydrocannabinol ( 1-10 micromol/l ) , anandamide ( 0.1-10 micromol/l ) and CP 55 , 940 ( 5 nmol/l to 1 micromol/l ) ) , nor the specific CB1 and CB2 antagonists ( AM251 ( 10-500 nmol/l ) and AM630 ( 50 nmol/l to 1 micromol/l ) , respectively ) had a significant effect upon 3H-2-deoxy-D-glucose uptake by Caco-2 cells .
	manualset3
201868	12	417438	7	NULL	NULL	0	NULL	AM251 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We verified that neither the cannabinoid receptor agonists ( tetrahydrocannabinol ( 1-10 micromol/l ) , anandamide ( 0.1-10 micromol/l ) and CP 55 , 940 ( 5 nmol/l to 1 micromol/l ) ) , nor the specific CB1 and CB2 antagonists ( AM251 ( 10-500 nmol/l ) and AM630 ( 50 nmol/l to 1 micromol/l ) , respectively ) had a significant effect upon 3H-2-deoxy-D-glucose uptake by Caco-2 cells .
	manualset3
201869	13	417438	7	NULL	NULL	0	NULL	10-500 nmol/l 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	We verified that neither the cannabinoid receptor agonists ( tetrahydrocannabinol ( 1-10 micromol/l ) , anandamide ( 0.1-10 micromol/l ) and CP 55 , 940 ( 5 nmol/l to 1 micromol/l ) ) , nor the specific CB1 and CB2 antagonists ( AM251 ( 10-500 nmol/l ) and AM630 ( 50 nmol/l to 1 micromol/l ) , respectively ) had a significant effect upon 3H-2-deoxy-D-glucose uptake by Caco-2 cells .
	manualset3
201870	14	417438	7	NULL	NULL	0	NULL	AM630	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We verified that neither the cannabinoid receptor agonists ( tetrahydrocannabinol ( 1-10 micromol/l ) , anandamide ( 0.1-10 micromol/l ) and CP 55 , 940 ( 5 nmol/l to 1 micromol/l ) ) , nor the specific CB1 and CB2 antagonists ( AM251 ( 10-500 nmol/l ) and AM630 ( 50 nmol/l to 1 micromol/l ) , respectively ) had a significant effect upon 3H-2-deoxy-D-glucose uptake by Caco-2 cells .
	manualset3
201871	15	417438	7	NULL	NULL	0	NULL	50 nmol/l to 1 micromol/l 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	We verified that neither the cannabinoid receptor agonists ( tetrahydrocannabinol ( 1-10 micromol/l ) , anandamide ( 0.1-10 micromol/l ) and CP 55 , 940 ( 5 nmol/l to 1 micromol/l ) ) , nor the specific CB1 and CB2 antagonists ( AM251 ( 10-500 nmol/l ) and AM630 ( 50 nmol/l to 1 micromol/l ) , respectively ) had a significant effect upon 3H-2-deoxy-D-glucose uptake by Caco-2 cells .
	manualset3
201872	16	417438	7	NULL	NULL	0	NULL	3H-2-deoxy-D-glucose uptake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We verified that neither the cannabinoid receptor agonists ( tetrahydrocannabinol ( 1-10 micromol/l ) , anandamide ( 0.1-10 micromol/l ) and CP 55 , 940 ( 5 nmol/l to 1 micromol/l ) ) , nor the specific CB1 and CB2 antagonists ( AM251 ( 10-500 nmol/l ) and AM630 ( 50 nmol/l to 1 micromol/l ) , respectively ) had a significant effect upon 3H-2-deoxy-D-glucose uptake by Caco-2 cells .
	manualset3
201873	17	417438	7	NULL	NULL	0	NULL	Caco-2 cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We verified that neither the cannabinoid receptor agonists ( tetrahydrocannabinol ( 1-10 micromol/l ) , anandamide ( 0.1-10 micromol/l ) and CP 55 , 940 ( 5 nmol/l to 1 micromol/l ) ) , nor the specific CB1 and CB2 antagonists ( AM251 ( 10-500 nmol/l ) and AM630 ( 50 nmol/l to 1 micromol/l ) , respectively ) had a significant effect upon 3H-2-deoxy-D-glucose uptake by Caco-2 cells .
	manualset3
201874	1	417439	7	NULL	NULL	0	NULL	major trends	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We were able to summarise the major trends in leaf shape variation using a principal components ( PC ) analysis and assess the changes in size , width and tip-to-base asymmetry within our leaf library .
	manualset3
201875	2	417439	7	NULL	NULL	0	NULL	leaf shape variation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We were able to summarise the major trends in leaf shape variation using a principal components ( PC ) analysis and assess the changes in size , width and tip-to-base asymmetry within our leaf library .
	manualset3
201876	3	417439	7	NULL	NULL	NULL	NULL	principal components ( PC ) analysis 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We were able to summarise the major trends in leaf shape variation using a principal components ( PC ) analysis and assess the changes in size , width and tip-to-base asymmetry within our leaf library .
	manualset3
201877	4	417439	7	NULL	NULL	0	NULL	changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We were able to summarise the major trends in leaf shape variation using a principal components ( PC ) analysis and assess the changes in size , width and tip-to-base asymmetry within our leaf library .
	manualset3
201878	5	417439	7	NULL	NULL	0	NULL	size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We were able to summarise the major trends in leaf shape variation using a principal components ( PC ) analysis and assess the changes in size , width and tip-to-base asymmetry within our leaf library .
	manualset3
201879	6	417439	7	NULL	NULL	0	NULL	 width	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We were able to summarise the major trends in leaf shape variation using a principal components ( PC ) analysis and assess the changes in size , width and tip-to-base asymmetry within our leaf library .
	manualset3
201880	7	417439	7	NULL	NULL	0	NULL	tip-to-base asymmetry	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We were able to summarise the major trends in leaf shape variation using a principal components ( PC ) analysis and assess the changes in size , width and tip-to-base asymmetry within our leaf library .
	manualset3
201881	8	417439	7	NULL	NULL	NULL	NULL	leaf library	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We were able to summarise the major trends in leaf shape variation using a principal components ( PC ) analysis and assess the changes in size , width and tip-to-base asymmetry within our leaf library .
	manualset3
201882	1	417440	7	NULL	NULL	0	NULL	components	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We were not able to demonstrate that components identified in vitro were associated with reduced aflatoxin accumulation in the field .
	manualset3
201883	2	417440	7	NULL	NULL	0	NULL	reduced aflatoxin accumulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We were not able to demonstrate that components identified in vitro were associated with reduced aflatoxin accumulation in the field .
	manualset3
201884	3	417440	7	NULL	NULL	0	NULL	field	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	We were not able to demonstrate that components identified in vitro were associated with reduced aflatoxin accumulation in the field .
	manualset3
201885	1	417441	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We will discuss the effects prolonged task performance on the behavioural and physiological indices of action monitoring , as well as the relationship between fatigue , motivation and individual differences .
	manualset3
201886	2	417441	7	NULL	NULL	0	NULL	prolonged task performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We will discuss the effects prolonged task performance on the behavioural and physiological indices of action monitoring , as well as the relationship between fatigue , motivation and individual differences .
	manualset3
201887	3	417441	7	NULL	NULL	0	NULL	behavioural indices	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We will discuss the effects prolonged task performance on the behavioural and physiological indices of action monitoring , as well as the relationship between fatigue , motivation and individual differences .
	manualset3
201888	4	417441	7	NULL	NULL	0	NULL	physiological indices	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We will discuss the effects prolonged task performance on the behavioural and physiological indices of action monitoring , as well as the relationship between fatigue , motivation and individual differences .
	manualset3
201889	5	417441	7	NULL	NULL	0	NULL	action monitoring	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We will discuss the effects prolonged task performance on the behavioural and physiological indices of action monitoring , as well as the relationship between fatigue , motivation and individual differences .
	manualset3
201890	6	417441	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	We will discuss the effects prolonged task performance on the behavioural and physiological indices of action monitoring , as well as the relationship between fatigue , motivation and individual differences .
	manualset3
201891	7	417441	7	NULL	NULL	0	NULL	fatigue	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We will discuss the effects prolonged task performance on the behavioural and physiological indices of action monitoring , as well as the relationship between fatigue , motivation and individual differences .
	manualset3
201892	8	417441	7	NULL	NULL	0	NULL	 motivation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We will discuss the effects prolonged task performance on the behavioural and physiological indices of action monitoring , as well as the relationship between fatigue , motivation and individual differences .
	manualset3
201893	9	417441	7	NULL	NULL	0	NULL	individual differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	We will discuss the effects prolonged task performance on the behavioural and physiological indices of action monitoring , as well as the relationship between fatigue , motivation and individual differences .
	manualset3
201894	1	417442	7	NULL	NULL	0	NULL	significance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We will discuss the significance of this tissue-specific localization with regard to phototransduction .
	manualset3
201895	2	417442	7	NULL	NULL	0	NULL	tissue-specific localization 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	We will discuss the significance of this tissue-specific localization with regard to phototransduction .
	manualset3
201896	3	417442	7	NULL	NULL	0	NULL	phototransduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We will discuss the significance of this tissue-specific localization with regard to phototransduction .
	manualset3
201897	1	417443	7	NULL	NULL	0	NULL	correlations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Weak but statistically significant correlations between DNA-strand breaks and motility/morphology parameters of sperm samples were observed in the neutral version of the COMET assay , while correlations between the same variables were statistically not significant in the alkaline version .
	manualset3
201898	2	417443	7	NULL	NULL	0	NULL	DNA-strand breaks	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Weak but statistically significant correlations between DNA-strand breaks and motility/morphology parameters of sperm samples were observed in the neutral version of the COMET assay , while correlations between the same variables were statistically not significant in the alkaline version .
	manualset3
201899	3	417443	7	NULL	NULL	0	NULL	motility/morphology parameters 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Weak but statistically significant correlations between DNA-strand breaks and motility/morphology parameters of sperm samples were observed in the neutral version of the COMET assay , while correlations between the same variables were statistically not significant in the alkaline version .
	manualset3
201900	4	417443	7	NULL	NULL	0	NULL	sperm samples	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Weak but statistically significant correlations between DNA-strand breaks and motility/morphology parameters of sperm samples were observed in the neutral version of the COMET assay , while correlations between the same variables were statistically not significant in the alkaline version .
	manualset3
201901	5	417443	7	NULL	NULL	0	NULL	neutral version	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Weak but statistically significant correlations between DNA-strand breaks and motility/morphology parameters of sperm samples were observed in the neutral version of the COMET assay , while correlations between the same variables were statistically not significant in the alkaline version .
	manualset3
201902	6	417443	7	NULL	NULL	0	NULL	COMET assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Weak but statistically significant correlations between DNA-strand breaks and motility/morphology parameters of sperm samples were observed in the neutral version of the COMET assay , while correlations between the same variables were statistically not significant in the alkaline version .
	manualset3
201903	7	417443	7	NULL	NULL	0	NULL	correlations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Weak but statistically significant correlations between DNA-strand breaks and motility/morphology parameters of sperm samples were observed in the neutral version of the COMET assay , while correlations between the same variables were statistically not significant in the alkaline version .
	manualset3
201904	8	417443	7	NULL	NULL	0	NULL	variables	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Weak but statistically significant correlations between DNA-strand breaks and motility/morphology parameters of sperm samples were observed in the neutral version of the COMET assay , while correlations between the same variables were statistically not significant in the alkaline version .
	manualset3
201905	9	417443	7	NULL	NULL	0	NULL	alkaline version	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Weak but statistically significant correlations between DNA-strand breaks and motility/morphology parameters of sperm samples were observed in the neutral version of the COMET assay , while correlations between the same variables were statistically not significant in the alkaline version .
	manualset3
201906	1	417444	7	NULL	NULL	0	NULL	experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Weakened by the experience , patients feel ageing .
	manualset3
201907	2	417444	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Weakened by the experience , patients feel ageing .
	manualset3
201908	3	417444	7	NULL	NULL	0	NULL	ageing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Weakened by the experience , patients feel ageing .
	manualset3
201909	1	417445	7	NULL	NULL	0	NULL	isolates	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All isolates were also growing on polymyxin-egg yolk-mannitol-bromothymol blue agar ( PEMBA ) ; however , 11 % isolates indicated that they did produce acid from mannitol , and 15 % isolates did not show any lecithinase activity .
	manualset3
201910	2	417445	7	NULL	NULL	0	NULL	polymyxin-egg yolk-mannitol-bromothymol blue agar ( PEMBA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All isolates were also growing on polymyxin-egg yolk-mannitol-bromothymol blue agar ( PEMBA ) ; however , 11 % isolates indicated that they did produce acid from mannitol , and 15 % isolates did not show any lecithinase activity .
	manualset3
201911	3	417445	7	NULL	NULL	0	NULL	11 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All isolates were also growing on polymyxin-egg yolk-mannitol-bromothymol blue agar ( PEMBA ) ; however , 11 % isolates indicated that they did produce acid from mannitol , and 15 % isolates did not show any lecithinase activity .
	manualset3
201912	4	417445	7	NULL	NULL	0	NULL	isolates	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All isolates were also growing on polymyxin-egg yolk-mannitol-bromothymol blue agar ( PEMBA ) ; however , 11 % isolates indicated that they did produce acid from mannitol , and 15 % isolates did not show any lecithinase activity .
	manualset3
201913	5	417445	7	NULL	NULL	0	NULL	acid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All isolates were also growing on polymyxin-egg yolk-mannitol-bromothymol blue agar ( PEMBA ) ; however , 11 % isolates indicated that they did produce acid from mannitol , and 15 % isolates did not show any lecithinase activity .
	manualset3
201914	6	417445	7	NULL	NULL	0	NULL	mannitol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All isolates were also growing on polymyxin-egg yolk-mannitol-bromothymol blue agar ( PEMBA ) ; however , 11 % isolates indicated that they did produce acid from mannitol , and 15 % isolates did not show any lecithinase activity .
	manualset3
201915	7	417445	7	NULL	NULL	0	NULL	15 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All isolates were also growing on polymyxin-egg yolk-mannitol-bromothymol blue agar ( PEMBA ) ; however , 11 % isolates indicated that they did produce acid from mannitol , and 15 % isolates did not show any lecithinase activity .
	manualset3
201916	8	417445	7	NULL	NULL	0	NULL	isolates	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All isolates were also growing on polymyxin-egg yolk-mannitol-bromothymol blue agar ( PEMBA ) ; however , 11 % isolates indicated that they did produce acid from mannitol , and 15 % isolates did not show any lecithinase activity .
	manualset3
201917	9	417445	7	NULL	NULL	0	NULL	lecithinase activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All isolates were also growing on polymyxin-egg yolk-mannitol-bromothymol blue agar ( PEMBA ) ; however , 11 % isolates indicated that they did produce acid from mannitol , and 15 % isolates did not show any lecithinase activity .
	manualset3
201918	1	417446	7	NULL	NULL	0	NULL	positive correlations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Weaker but still positive correlations are found for crab and D. pumilio conspecific visual perception , while frog coloration as viewed by snakes is not related to toxicity .
	manualset3
201919	2	417446	7	NULL	NULL	0	NULL	crab	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Weaker but still positive correlations are found for crab and D. pumilio conspecific visual perception , while frog coloration as viewed by snakes is not related to toxicity .
	manualset3
201920	3	417446	7	NULL	NULL	0	NULL	D. pumilio conspecific visual perception	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Weaker but still positive correlations are found for crab and D. pumilio conspecific visual perception , while frog coloration as viewed by snakes is not related to toxicity .
	manualset3
201921	4	417446	7	NULL	NULL	0	NULL	frog coloration 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Weaker but still positive correlations are found for crab and D. pumilio conspecific visual perception , while frog coloration as viewed by snakes is not related to toxicity .
	manualset3
201922	5	417446	7	NULL	NULL	0	NULL	snakes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Weaker but still positive correlations are found for crab and D. pumilio conspecific visual perception , while frog coloration as viewed by snakes is not related to toxicity .
	manualset3
201923	6	417446	7	NULL	NULL	0	NULL	toxicity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Weaker but still positive correlations are found for crab and D. pumilio conspecific visual perception , while frog coloration as viewed by snakes is not related to toxicity .
	manualset3
201924	1	417447	7	NULL	NULL	0	NULL	 TRPA1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Weakly acidic , but strongly irritating : TRPA1 and the activation of nociceptors by cytoplasmic acidification .
	manualset3
201925	2	417447	7	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Weakly acidic , but strongly irritating : TRPA1 and the activation of nociceptors by cytoplasmic acidification .
	manualset3
201926	3	417447	7	NULL	NULL	0	NULL	nociceptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Weakly acidic , but strongly irritating : TRPA1 and the activation of nociceptors by cytoplasmic acidification .
	manualset3
201927	4	417447	7	NULL	NULL	0	NULL	cytoplasmic acidification	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Weakly acidic , but strongly irritating : TRPA1 and the activation of nociceptors by cytoplasmic acidification .
	manualset3
201928	1	417448	7	NULL	NULL	0	NULL	Weakness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Weakness of the lumbar extensors was clearly shown by isokinetic measurement and a marked atrophy of these muscles with fatty infiltration was demonstrated by CT scanning .
	manualset3
201929	2	417448	7	NULL	NULL	0	NULL	lumbar extensors	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Weakness of the lumbar extensors was clearly shown by isokinetic measurement and a marked atrophy of these muscles with fatty infiltration was demonstrated by CT scanning .
	manualset3
201930	3	417448	7	NULL	NULL	0	NULL	 isokinetic measurement	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Weakness of the lumbar extensors was clearly shown by isokinetic measurement and a marked atrophy of these muscles with fatty infiltration was demonstrated by CT scanning .
	manualset3
201931	4	417448	7	NULL	NULL	0	NULL	atrophy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Weakness of the lumbar extensors was clearly shown by isokinetic measurement and a marked atrophy of these muscles with fatty infiltration was demonstrated by CT scanning .
	manualset3
201932	5	417448	7	NULL	NULL	0	NULL	 muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Weakness of the lumbar extensors was clearly shown by isokinetic measurement and a marked atrophy of these muscles with fatty infiltration was demonstrated by CT scanning .
	manualset3
201933	6	417448	7	NULL	NULL	0	NULL	fatty infiltration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Weakness of the lumbar extensors was clearly shown by isokinetic measurement and a marked atrophy of these muscles with fatty infiltration was demonstrated by CT scanning .
	manualset3
201934	7	417448	7	NULL	NULL	0	NULL	 CT scanning	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Weakness of the lumbar extensors was clearly shown by isokinetic measurement and a marked atrophy of these muscles with fatty infiltration was demonstrated by CT scanning .
	manualset3
201935	1	417449	7	NULL	NULL	0	NULL	Wear characteristics 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Wear characteristics of sliding pairs of zirconia ( Y-TZP ) for hip endoprostheses .
	manualset3
201936	2	417449	7	NULL	NULL	0	NULL	 sliding pairs	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Wear characteristics of sliding pairs of zirconia ( Y-TZP ) for hip endoprostheses .
	manualset3
201937	3	417449	7	NULL	NULL	NULL	NULL	 zirconia ( Y-TZP )	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Wear characteristics of sliding pairs of zirconia ( Y-TZP ) for hip endoprostheses .
	manualset3
201938	4	417449	7	NULL	NULL	0	NULL	hip endoprostheses	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Wear characteristics of sliding pairs of zirconia ( Y-TZP ) for hip endoprostheses .
	manualset3
201939	1	417450	7	NULL	NULL	0	NULL	Weight 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Weight , but neither height nor age , was significant for head BMD .
	manualset3
201940	2	417450	7	NULL	NULL	0	NULL	height 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Weight , but neither height nor age , was significant for head BMD .
	manualset3
201941	3	417450	7	NULL	NULL	0	NULL	age	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Weight , but neither height nor age , was significant for head BMD .
	manualset3
201942	4	417450	7	NULL	NULL	0	NULL	head BMD	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Weight , but neither height nor age , was significant for head BMD .
	manualset3
201943	1	417451	7	NULL	NULL	0	NULL	Weight gain	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Weight gain , through typical Western diet ; limited levels of activity ; and , more recently , stress-related changes in neuroendocrine function may lead to insulin resistance and hyperinsulinemia .
	manualset3
201944	2	417451	7	NULL	NULL	NULL	NULL	Western diet	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Weight gain , through typical Western diet ; limited levels of activity ; and , more recently , stress-related changes in neuroendocrine function may lead to insulin resistance and hyperinsulinemia .
	manualset3
201945	3	417451	7	NULL	NULL	0	NULL	limited levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Weight gain , through typical Western diet ; limited levels of activity ; and , more recently , stress-related changes in neuroendocrine function may lead to insulin resistance and hyperinsulinemia .
	manualset3
201946	4	417451	7	NULL	NULL	0	NULL	 activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Weight gain , through typical Western diet ; limited levels of activity ; and , more recently , stress-related changes in neuroendocrine function may lead to insulin resistance and hyperinsulinemia .
	manualset3
201947	5	417451	7	NULL	NULL	0	NULL	 stress-related changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Weight gain , through typical Western diet ; limited levels of activity ; and , more recently , stress-related changes in neuroendocrine function may lead to insulin resistance and hyperinsulinemia .
	manualset3
201948	6	417451	7	NULL	NULL	0	NULL	neuroendocrine function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Weight gain , through typical Western diet ; limited levels of activity ; and , more recently , stress-related changes in neuroendocrine function may lead to insulin resistance and hyperinsulinemia .
	manualset3
201949	7	417451	7	NULL	NULL	0	NULL	insulin resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Weight gain , through typical Western diet ; limited levels of activity ; and , more recently , stress-related changes in neuroendocrine function may lead to insulin resistance and hyperinsulinemia .
	manualset3
201950	8	417451	7	NULL	NULL	0	NULL	hyperinsulinemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Weight gain , through typical Western diet ; limited levels of activity ; and , more recently , stress-related changes in neuroendocrine function may lead to insulin resistance and hyperinsulinemia .
	manualset3
201951	1	417452	7	NULL	NULL	0	NULL	Weight loss	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Weight loss in an online weight control program was related to dynamic Web features that provided feedback , support , and motivation to participants .
	manualset3
201952	2	417452	7	NULL	NULL	NULL	NULL	online weight control program	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Weight loss in an online weight control program was related to dynamic Web features that provided feedback , support , and motivation to participants .
	manualset3
201953	3	417452	7	NULL	NULL	0	NULL	dynamic Web features	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Weight loss in an online weight control program was related to dynamic Web features that provided feedback , support , and motivation to participants .
	manualset3
201954	4	417452	7	NULL	NULL	0	NULL	feedback	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Weight loss in an online weight control program was related to dynamic Web features that provided feedback , support , and motivation to participants .
	manualset3
201955	5	417452	7	NULL	NULL	0	NULL	support	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Weight loss in an online weight control program was related to dynamic Web features that provided feedback , support , and motivation to participants .
	manualset3
201956	6	417452	7	NULL	NULL	0	NULL	motivation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Weight loss in an online weight control program was related to dynamic Web features that provided feedback , support , and motivation to participants .
	manualset3
201957	7	417452	7	NULL	NULL	0	NULL	participants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Weight loss in an online weight control program was related to dynamic Web features that provided feedback , support , and motivation to participants .
	manualset3
201958	1	417453	7	NULL	NULL	0	NULL	Weight loss	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Weight loss predicts mortality after recurrent oral cavity and oropharyngeal carcinomas .
	manualset3
201959	2	417453	7	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Weight loss predicts mortality after recurrent oral cavity and oropharyngeal carcinomas .
	manualset3
201960	3	417453	7	NULL	NULL	0	NULL	recurrent oral cavity carcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Weight loss predicts mortality after recurrent oral cavity and oropharyngeal carcinomas .
	manualset3
201961	4	417453	7	NULL	NULL	0	NULL	oropharyngeal carcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Weight loss predicts mortality after recurrent oral cavity and oropharyngeal carcinomas .
	manualset3
201962	1	417454	7	NULL	NULL	0	NULL	Weights	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Weights had quite modest effects on point estimates of prevalences but resulted in major increases in variance unless trimmed .
	manualset3
201963	2	417454	7	NULL	NULL	0	NULL	modest effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Weights had quite modest effects on point estimates of prevalences but resulted in major increases in variance unless trimmed .
	manualset3
201964	3	417454	7	NULL	NULL	0	NULL	 point estimates	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Weights had quite modest effects on point estimates of prevalences but resulted in major increases in variance unless trimmed .
	manualset3
201965	4	417454	7	NULL	NULL	0	NULL	variance	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Weights had quite modest effects on point estimates of prevalences but resulted in major increases in variance unless trimmed .
	manualset3
204482	5	417454	7	NULL	NULL	0	NULL	prevalences 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Weights had quite modest effects on point estimates of prevalences but resulted in major increases in variance unless trimmed .
	manualset3
204483	6	417454	7	NULL	NULL	0	NULL	major increases	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Weights had quite modest effects on point estimates of prevalences but resulted in major increases in variance unless trimmed .
	manualset3
201966	1	417455	7	NULL	NULL	0	NULL	Wellmer , K. Fuchs , and P. Vlker 	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	Wellmer , K. Fuchs , and P. Vlker : `` Gastric resection in severe hemophilia A during substitution with porcine antihemophilic globulin '' .
	manualset3
201967	2	417455	7	NULL	NULL	0	NULL	Gastric resection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Wellmer , K. Fuchs , and P. Vlker : `` Gastric resection in severe hemophilia A during substitution with porcine antihemophilic globulin '' .
	manualset3
201968	3	417455	7	NULL	NULL	0	NULL	severe hemophilia A	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Wellmer , K. Fuchs , and P. Vlker : `` Gastric resection in severe hemophilia A during substitution with porcine antihemophilic globulin '' .
	manualset3
201969	4	417455	7	NULL	NULL	0	NULL	substitution	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Wellmer , K. Fuchs , and P. Vlker : `` Gastric resection in severe hemophilia A during substitution with porcine antihemophilic globulin '' .
	manualset3
201970	5	417455	7	NULL	NULL	0	NULL	 porcine antihemophilic globulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Wellmer , K. Fuchs , and P. Vlker : `` Gastric resection in severe hemophilia A during substitution with porcine antihemophilic globulin '' .
	manualset3
201971	1	417456	7	NULL	NULL	0	NULL	 lambs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	All lambs showed significant increase in bone marrow EpoR mRNA levels after phlebotomy-induced anemia .
	manualset3
201972	2	417456	7	NULL	NULL	0	NULL	bone marrow EpoR mRNA levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All lambs showed significant increase in bone marrow EpoR mRNA levels after phlebotomy-induced anemia .
	manualset3
201973	3	417456	7	NULL	NULL	0	NULL	phlebotomy-induced anemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	All lambs showed significant increase in bone marrow EpoR mRNA levels after phlebotomy-induced anemia .
	manualset3
204484	4	417456	7	NULL	NULL	0	NULL	increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All lambs showed significant increase in bone marrow EpoR mRNA levels after phlebotomy-induced anemia .
	manualset3
201974	1	417457	7	NULL	NULL	0	NULL	Western blot analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis indicated that phosphorylation of Erk1/2 , a protein downstream of Ras , was increased by propiconazole .
	manualset3
201975	2	417457	7	NULL	NULL	0	NULL	phosphorylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis indicated that phosphorylation of Erk1/2 , a protein downstream of Ras , was increased by propiconazole .
	manualset3
201976	3	417457	7	NULL	NULL	0	NULL	Erk1/2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis indicated that phosphorylation of Erk1/2 , a protein downstream of Ras , was increased by propiconazole .
	manualset3
201977	4	417457	7	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis indicated that phosphorylation of Erk1/2 , a protein downstream of Ras , was increased by propiconazole .
	manualset3
201978	5	417457	7	NULL	NULL	0	NULL	Ras	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis indicated that phosphorylation of Erk1/2 , a protein downstream of Ras , was increased by propiconazole .
	manualset3
201979	6	417457	7	NULL	NULL	0	NULL	propiconazole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis indicated that phosphorylation of Erk1/2 , a protein downstream of Ras , was increased by propiconazole .
	manualset3
201980	1	417458	7	NULL	NULL	0	NULL	Western blot analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis revealed high VEGF expressors ( tumour/normal tissue density ) / = 3-fold ) in 26 patients ( 43 % ) and low VEGF expressors ( & lt ; 3-fold ) in 34 patients ( 57 % ) .
	manualset3
201981	2	417458	7	NULL	NULL	0	NULL	high VEGF expressors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis revealed high VEGF expressors ( tumour/normal tissue density ) / = 3-fold ) in 26 patients ( 43 % ) and low VEGF expressors ( & lt ; 3-fold ) in 34 patients ( 57 % ) .
	manualset3
201982	3	417458	7	NULL	NULL	0	NULL	tumour/normal tissue density 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis revealed high VEGF expressors ( tumour/normal tissue density ) / = 3-fold ) in 26 patients ( 43 % ) and low VEGF expressors ( & lt ; 3-fold ) in 34 patients ( 57 % ) .
	manualset3
201983	4	417458	7	NULL	NULL	0	NULL	3-fold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis revealed high VEGF expressors ( tumour/normal tissue density ) / = 3-fold ) in 26 patients ( 43 % ) and low VEGF expressors ( & lt ; 3-fold ) in 34 patients ( 57 % ) .
	manualset3
201984	5	417458	7	NULL	NULL	0	NULL	26 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis revealed high VEGF expressors ( tumour/normal tissue density ) / = 3-fold ) in 26 patients ( 43 % ) and low VEGF expressors ( & lt ; 3-fold ) in 34 patients ( 57 % ) .
	manualset3
201985	6	417458	7	NULL	NULL	0	NULL	43 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis revealed high VEGF expressors ( tumour/normal tissue density ) / = 3-fold ) in 26 patients ( 43 % ) and low VEGF expressors ( & lt ; 3-fold ) in 34 patients ( 57 % ) .
	manualset3
201986	7	417458	7	NULL	NULL	0	NULL	low VEGF expressors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis revealed high VEGF expressors ( tumour/normal tissue density ) / = 3-fold ) in 26 patients ( 43 % ) and low VEGF expressors ( & lt ; 3-fold ) in 34 patients ( 57 % ) .
	manualset3
201987	8	417458	7	NULL	NULL	0	NULL	& lt ; 3-fold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis revealed high VEGF expressors ( tumour/normal tissue density ) / = 3-fold ) in 26 patients ( 43 % ) and low VEGF expressors ( & lt ; 3-fold ) in 34 patients ( 57 % ) .
	manualset3
201988	9	417458	7	NULL	NULL	0	NULL	34 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis revealed high VEGF expressors ( tumour/normal tissue density ) / = 3-fold ) in 26 patients ( 43 % ) and low VEGF expressors ( & lt ; 3-fold ) in 34 patients ( 57 % ) .
	manualset3
201989	10	417458	7	NULL	NULL	0	NULL	57 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis revealed high VEGF expressors ( tumour/normal tissue density ) / = 3-fold ) in 26 patients ( 43 % ) and low VEGF expressors ( & lt ; 3-fold ) in 34 patients ( 57 % ) .
	manualset3
201990	1	417459	7	NULL	NULL	0	NULL	Western blot analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis revealed that the expression of phosphorylated protein kinase C ( p-PKC ) and phosphorylated extracellular signal-regulated kinase ( p-ERK1 / 2 ) was increased in the liver of treated animals .
	manualset3
201991	2	417459	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis revealed that the expression of phosphorylated protein kinase C ( p-PKC ) and phosphorylated extracellular signal-regulated kinase ( p-ERK1 / 2 ) was increased in the liver of treated animals .
	manualset3
201992	3	417459	7	NULL	NULL	0	NULL	phosphorylated protein kinase C ( p-PKC )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis revealed that the expression of phosphorylated protein kinase C ( p-PKC ) and phosphorylated extracellular signal-regulated kinase ( p-ERK1 / 2 ) was increased in the liver of treated animals .
	manualset3
201993	4	417459	7	NULL	NULL	0	NULL	phosphorylated extracellular signal-regulated kinase ( p-ERK1 / 2 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis revealed that the expression of phosphorylated protein kinase C ( p-PKC ) and phosphorylated extracellular signal-regulated kinase ( p-ERK1 / 2 ) was increased in the liver of treated animals .
	manualset3
201994	5	417459	7	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis revealed that the expression of phosphorylated protein kinase C ( p-PKC ) and phosphorylated extracellular signal-regulated kinase ( p-ERK1 / 2 ) was increased in the liver of treated animals .
	manualset3
201995	6	417459	7	NULL	NULL	0	NULL	treated animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis revealed that the expression of phosphorylated protein kinase C ( p-PKC ) and phosphorylated extracellular signal-regulated kinase ( p-ERK1 / 2 ) was increased in the liver of treated animals .
	manualset3
201996	1	417460	7	NULL	NULL	0	NULL	Western blot analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis showed that ATL-1 increased HO-1 protein expression associated with increased mRNA levels on EC in a time - and concentration-dependent fashion .
	manualset3
201997	2	417460	7	NULL	NULL	0	NULL	ATL-1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis showed that ATL-1 increased HO-1 protein expression associated with increased mRNA levels on EC in a time - and concentration-dependent fashion .
	manualset3
201998	3	417460	7	NULL	NULL	NULL	NULL	HO-1 protein expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Western blot analysis showed that ATL-1 increased HO-1 protein expression associated with increased mRNA levels on EC in a time - and concentration-dependent fashion .
	manualset3
201999	4	417460	7	NULL	NULL	0	NULL	increased mRNA levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis showed that ATL-1 increased HO-1 protein expression associated with increased mRNA levels on EC in a time - and concentration-dependent fashion .
	manualset3
202000	5	417460	7	NULL	NULL	0	NULL	EC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis showed that ATL-1 increased HO-1 protein expression associated with increased mRNA levels on EC in a time - and concentration-dependent fashion .
	manualset3
202001	6	417460	7	NULL	NULL	0	NULL	time - dependent fashion	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis showed that ATL-1 increased HO-1 protein expression associated with increased mRNA levels on EC in a time - and concentration-dependent fashion .
	manualset3
202002	7	417460	7	NULL	NULL	0	NULL	concentration-dependent fashion	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis showed that ATL-1 increased HO-1 protein expression associated with increased mRNA levels on EC in a time - and concentration-dependent fashion .
	manualset3
202003	1	417461	7	NULL	NULL	0	NULL	Western blot analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis showed that atypical PKC was activated by LNO ( 2 ) stimulation , with PKC and Erk activation also demonstrated in primary culture of human lung type II cells .
	manualset3
202004	2	417461	7	NULL	NULL	0	NULL	atypical PKC 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis showed that atypical PKC was activated by LNO ( 2 ) stimulation , with PKC and Erk activation also demonstrated in primary culture of human lung type II cells .
	manualset3
202005	3	417461	7	NULL	NULL	0	NULL	LNO ( 2 ) stimulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis showed that atypical PKC was activated by LNO ( 2 ) stimulation , with PKC and Erk activation also demonstrated in primary culture of human lung type II cells .
	manualset3
202006	4	417461	7	NULL	NULL	0	NULL	PKC activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis showed that atypical PKC was activated by LNO ( 2 ) stimulation , with PKC and Erk activation also demonstrated in primary culture of human lung type II cells .
	manualset3
202007	5	417461	7	NULL	NULL	0	NULL	Erk activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis showed that atypical PKC was activated by LNO ( 2 ) stimulation , with PKC and Erk activation also demonstrated in primary culture of human lung type II cells .
	manualset3
202008	6	417461	7	NULL	NULL	0	NULL	primary culture 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis showed that atypical PKC was activated by LNO ( 2 ) stimulation , with PKC and Erk activation also demonstrated in primary culture of human lung type II cells .
	manualset3
202009	7	417461	7	NULL	NULL	0	NULL	human lung type II cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis showed that atypical PKC was activated by LNO ( 2 ) stimulation , with PKC and Erk activation also demonstrated in primary culture of human lung type II cells .
	manualset3
202010	1	417462	7	NULL	NULL	0	NULL	Western blot analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis showed that the protein level of CTRP3/cartducin was also increased in these two osteosarcoma cell lines .
	manualset3
202011	2	417462	7	NULL	NULL	0	NULL	 protein level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis showed that the protein level of CTRP3/cartducin was also increased in these two osteosarcoma cell lines .
	manualset3
202012	3	417462	7	NULL	NULL	0	NULL	CTRP3/cartducin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis showed that the protein level of CTRP3/cartducin was also increased in these two osteosarcoma cell lines .
	manualset3
202013	4	417462	7	NULL	NULL	0	NULL	two osteosarcoma cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis showed that the protein level of CTRP3/cartducin was also increased in these two osteosarcoma cell lines .
	manualset3
202014	1	417463	7	NULL	NULL	0	NULL	Western blot analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis showed that the size and the expression level of mutant AR in transfected cells were comparable to the wild type .
	manualset3
202015	2	417463	7	NULL	NULL	0	NULL	size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis showed that the size and the expression level of mutant AR in transfected cells were comparable to the wild type .
	manualset3
202016	3	417463	7	NULL	NULL	0	NULL	expression level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis showed that the size and the expression level of mutant AR in transfected cells were comparable to the wild type .
	manualset3
202017	4	417463	7	NULL	NULL	0	NULL	mutant AR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis showed that the size and the expression level of mutant AR in transfected cells were comparable to the wild type .
	manualset3
202018	5	417463	7	NULL	NULL	0	NULL	transfected cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis showed that the size and the expression level of mutant AR in transfected cells were comparable to the wild type .
	manualset3
202019	6	417463	7	NULL	NULL	0	NULL	wild type	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blot analysis showed that the size and the expression level of mutant AR in transfected cells were comparable to the wild type .
	manualset3
202020	1	417464	7	NULL	NULL	0	NULL	Western blots	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blots of total brain protein ( RIPA ) and sequential extraction buffers ( high salt , high salt/Triton X-100 , SDS and formic acid ) of increasing protein extraction strength were performed to examine solubility state .
	manualset3
202021	2	417464	7	NULL	NULL	0	NULL	total brain protein ( RIPA ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blots of total brain protein ( RIPA ) and sequential extraction buffers ( high salt , high salt/Triton X-100 , SDS and formic acid ) of increasing protein extraction strength were performed to examine solubility state .
	manualset3
202022	3	417464	7	NULL	NULL	0	NULL	sequential extraction buffers 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blots of total brain protein ( RIPA ) and sequential extraction buffers ( high salt , high salt/Triton X-100 , SDS and formic acid ) of increasing protein extraction strength were performed to examine solubility state .
	manualset3
202023	4	417464	7	NULL	NULL	0	NULL	high salt	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blots of total brain protein ( RIPA ) and sequential extraction buffers ( high salt , high salt/Triton X-100 , SDS and formic acid ) of increasing protein extraction strength were performed to examine solubility state .
	manualset3
202024	5	417464	7	NULL	NULL	0	NULL	high salt/Triton X-100	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blots of total brain protein ( RIPA ) and sequential extraction buffers ( high salt , high salt/Triton X-100 , SDS and formic acid ) of increasing protein extraction strength were performed to examine solubility state .
	manualset3
202025	6	417464	7	NULL	NULL	0	NULL	SDS	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blots of total brain protein ( RIPA ) and sequential extraction buffers ( high salt , high salt/Triton X-100 , SDS and formic acid ) of increasing protein extraction strength were performed to examine solubility state .
	manualset3
202026	7	417464	7	NULL	NULL	0	NULL	formic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blots of total brain protein ( RIPA ) and sequential extraction buffers ( high salt , high salt/Triton X-100 , SDS and formic acid ) of increasing protein extraction strength were performed to examine solubility state .
	manualset3
202027	8	417464	7	NULL	NULL	0	NULL	protein extraction strength	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blots of total brain protein ( RIPA ) and sequential extraction buffers ( high salt , high salt/Triton X-100 , SDS and formic acid ) of increasing protein extraction strength were performed to examine solubility state .
	manualset3
202028	9	417464	7	NULL	NULL	0	NULL	solubility state	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blots of total brain protein ( RIPA ) and sequential extraction buffers ( high salt , high salt/Triton X-100 , SDS and formic acid ) of increasing protein extraction strength were performed to examine solubility state .
	manualset3
202029	1	417465	7	NULL	NULL	0	NULL	Western blotting	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blotting and immunohistochemistry analyses were performed to validate the expression of a bottleneck phosphoprotein YAP1 in cancer cell lines and tissues .
	manualset3
202030	2	417465	7	NULL	NULL	0	NULL	immunohistochemistry analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blotting and immunohistochemistry analyses were performed to validate the expression of a bottleneck phosphoprotein YAP1 in cancer cell lines and tissues .
	manualset3
202031	3	417465	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blotting and immunohistochemistry analyses were performed to validate the expression of a bottleneck phosphoprotein YAP1 in cancer cell lines and tissues .
	manualset3
202032	4	417465	7	NULL	NULL	0	NULL	phosphoprotein YAP1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blotting and immunohistochemistry analyses were performed to validate the expression of a bottleneck phosphoprotein YAP1 in cancer cell lines and tissues .
	manualset3
202033	5	417465	7	NULL	NULL	0	NULL	cancer cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blotting and immunohistochemistry analyses were performed to validate the expression of a bottleneck phosphoprotein YAP1 in cancer cell lines and tissues .
	manualset3
202034	6	417465	7	NULL	NULL	0	NULL	tissues 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blotting and immunohistochemistry analyses were performed to validate the expression of a bottleneck phosphoprotein YAP1 in cancer cell lines and tissues .
	manualset3
202035	1	417466	7	NULL	NULL	0	NULL	Western blotting	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blotting of dormant spore and vegetative cell fractions separated by SDS-PAGE indicated that the 31 kDa enzyme is spore-specific and that the enzyme in the dormant spore exists as a 36 kDa protein which has no cortex-lytic activity .
	manualset3
202036	2	417466	7	NULL	NULL	0	NULL	dormant spore cell fractions	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blotting of dormant spore and vegetative cell fractions separated by SDS-PAGE indicated that the 31 kDa enzyme is spore-specific and that the enzyme in the dormant spore exists as a 36 kDa protein which has no cortex-lytic activity .
	manualset3
202037	3	417466	7	NULL	NULL	0	NULL	vegetative cell fractions	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blotting of dormant spore and vegetative cell fractions separated by SDS-PAGE indicated that the 31 kDa enzyme is spore-specific and that the enzyme in the dormant spore exists as a 36 kDa protein which has no cortex-lytic activity .
	manualset3
202038	4	417466	7	NULL	NULL	0	NULL	SDS-PAGE	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blotting of dormant spore and vegetative cell fractions separated by SDS-PAGE indicated that the 31 kDa enzyme is spore-specific and that the enzyme in the dormant spore exists as a 36 kDa protein which has no cortex-lytic activity .
	manualset3
202039	5	417466	7	NULL	NULL	0	NULL	31 kDa	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blotting of dormant spore and vegetative cell fractions separated by SDS-PAGE indicated that the 31 kDa enzyme is spore-specific and that the enzyme in the dormant spore exists as a 36 kDa protein which has no cortex-lytic activity .
	manualset3
202040	6	417466	7	NULL	NULL	NULL	NULL	enzyme	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Western blotting of dormant spore and vegetative cell fractions separated by SDS-PAGE indicated that the 31 kDa enzyme is spore-specific and that the enzyme in the dormant spore exists as a 36 kDa protein which has no cortex-lytic activity .
	manualset3
202041	7	417466	7	NULL	NULL	0	NULL	spore-specific	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blotting of dormant spore and vegetative cell fractions separated by SDS-PAGE indicated that the 31 kDa enzyme is spore-specific and that the enzyme in the dormant spore exists as a 36 kDa protein which has no cortex-lytic activity .
	manualset3
202042	8	417466	7	NULL	NULL	NULL	NULL	 enzyme	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Western blotting of dormant spore and vegetative cell fractions separated by SDS-PAGE indicated that the 31 kDa enzyme is spore-specific and that the enzyme in the dormant spore exists as a 36 kDa protein which has no cortex-lytic activity .
	manualset3
202043	9	417466	7	NULL	NULL	0	NULL	dormant spore	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blotting of dormant spore and vegetative cell fractions separated by SDS-PAGE indicated that the 31 kDa enzyme is spore-specific and that the enzyme in the dormant spore exists as a 36 kDa protein which has no cortex-lytic activity .
	manualset3
202044	10	417466	7	NULL	NULL	NULL	NULL	36 kDa protein	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Western blotting of dormant spore and vegetative cell fractions separated by SDS-PAGE indicated that the 31 kDa enzyme is spore-specific and that the enzyme in the dormant spore exists as a 36 kDa protein which has no cortex-lytic activity .
	manualset3
202045	11	417466	7	NULL	NULL	0	NULL	cortex-lytic activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blotting of dormant spore and vegetative cell fractions separated by SDS-PAGE indicated that the 31 kDa enzyme is spore-specific and that the enzyme in the dormant spore exists as a 36 kDa protein which has no cortex-lytic activity .
	manualset3
202046	1	417467	7	NULL	NULL	0	NULL	Western blotting	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blotting with a monoclonal antibody against gp46 was used to show that the expression of gp46 was normal in D-1 but was reduced in mutant C-8 compared with L6 .
	manualset3
202047	2	417467	7	NULL	NULL	0	NULL	monoclonal antibody 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blotting with a monoclonal antibody against gp46 was used to show that the expression of gp46 was normal in D-1 but was reduced in mutant C-8 compared with L6 .
	manualset3
202048	3	417467	7	NULL	NULL	0	NULL	 gp46	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blotting with a monoclonal antibody against gp46 was used to show that the expression of gp46 was normal in D-1 but was reduced in mutant C-8 compared with L6 .
	manualset3
202049	4	417467	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blotting with a monoclonal antibody against gp46 was used to show that the expression of gp46 was normal in D-1 but was reduced in mutant C-8 compared with L6 .
	manualset3
202050	5	417467	7	NULL	NULL	0	NULL	gp46	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Western blotting with a monoclonal antibody against gp46 was used to show that the expression of gp46 was normal in D-1 but was reduced in mutant C-8 compared with L6 .
	manualset3
202051	6	417467	7	NULL	NULL	NULL	NULL	D-1 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Western blotting with a monoclonal antibody against gp46 was used to show that the expression of gp46 was normal in D-1 but was reduced in mutant C-8 compared with L6 .
	manualset3
202052	7	417467	7	NULL	NULL	NULL	NULL	mutant C-8	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Western blotting with a monoclonal antibody against gp46 was used to show that the expression of gp46 was normal in D-1 but was reduced in mutant C-8 compared with L6 .
	manualset3
202053	8	417467	7	NULL	NULL	NULL	NULL	L6	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Western blotting with a monoclonal antibody against gp46 was used to show that the expression of gp46 was normal in D-1 but was reduced in mutant C-8 compared with L6 .
	manualset3
202054	1	417468	7	NULL	NULL	0	NULL	Western scrub-jays 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Western scrub-jays conceal auditory information when competitors can hear but can not see .
	manualset3
202055	2	417468	7	NULL	NULL	0	NULL	auditory information	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Western scrub-jays conceal auditory information when competitors can hear but can not see .
	manualset3
202056	3	417468	7	NULL	NULL	NULL	NULL	competitors	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Western scrub-jays conceal auditory information when competitors can hear but can not see .
	manualset3
202057	1	417469	7	NULL	NULL	0	NULL	examples	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	What are some examples of ICT capacity development programs in the Pacific Islands region ?
	manualset3
202058	2	417469	7	NULL	NULL	NULL	NULL	ICT capacity development programs	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	What are some examples of ICT capacity development programs in the Pacific Islands region ?
	manualset3
202059	3	417469	7	NULL	NULL	0	NULL	Pacific Islands region	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	What are some examples of ICT capacity development programs in the Pacific Islands region ?
	manualset3
202060	1	417470	7	NULL	NULL	0	NULL	determinants	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	What are the determinants of gene expression levels and breadths in the human genome ?
	manualset3
202061	2	417470	7	NULL	NULL	0	NULL	gene expression levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	What are the determinants of gene expression levels and breadths in the human genome ?
	manualset3
202062	3	417470	7	NULL	NULL	0	NULL	breadths	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	What are the determinants of gene expression levels and breadths in the human genome ?
	manualset3
202063	4	417470	7	NULL	NULL	0	NULL	human genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	What are the determinants of gene expression levels and breadths in the human genome ?
	manualset3
202064	1	417471	7	NULL	NULL	0	NULL	dentistry	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	What could it mean for dentistry ?
	manualset3
202065	1	417472	7	NULL	NULL	0	NULL	human factor	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	All leading to a growing interest in the human factor in industry , where the medical officer should help to shape a satisfied , rational and productive worker in a healthy work environment .
	manualset3
202066	2	417472	7	NULL	NULL	0	NULL	industry	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	All leading to a growing interest in the human factor in industry , where the medical officer should help to shape a satisfied , rational and productive worker in a healthy work environment .
	manualset3
202067	3	417472	7	NULL	NULL	0	NULL	medical officer	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	All leading to a growing interest in the human factor in industry , where the medical officer should help to shape a satisfied , rational and productive worker in a healthy work environment .
	manualset3
202068	4	417472	7	NULL	NULL	0	NULL	productive worker 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	All leading to a growing interest in the human factor in industry , where the medical officer should help to shape a satisfied , rational and productive worker in a healthy work environment .
	manualset3
202069	5	417472	7	NULL	NULL	0	NULL	healthy work environment	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	All leading to a growing interest in the human factor in industry , where the medical officer should help to shape a satisfied , rational and productive worker in a healthy work environment .
	manualset3
202070	1	417473	7	NULL	NULL	0	NULL	perceptual experience	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	What does perceptual experience contribute to figure-ground segregation ?
	manualset3
202071	2	417473	7	NULL	NULL	0	NULL	figure-ground segregation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	What does perceptual experience contribute to figure-ground segregation ?
	manualset3
202072	1	417474	7	NULL	NULL	0	NULL	Ecstasy 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	What is Ecstasy and what is the management of its toxicity in patients admitted to hospital ?
	manualset3
202073	2	417474	7	NULL	NULL	0	NULL	management 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	What is Ecstasy and what is the management of its toxicity in patients admitted to hospital ?
	manualset3
202074	3	417474	7	NULL	NULL	0	NULL	toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	What is Ecstasy and what is the management of its toxicity in patients admitted to hospital ?
	manualset3
202075	4	417474	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	What is Ecstasy and what is the management of its toxicity in patients admitted to hospital ?
	manualset3
202076	5	417474	7	NULL	NULL	0	NULL	hospital	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	What is Ecstasy and what is the management of its toxicity in patients admitted to hospital ?
	manualset3
202077	1	417475	7	NULL	NULL	0	NULL	 role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	What is said so far must not exclude the importance of recognizing the role of the internal urethral structures to maintain continence , in particular the quality of urethral muscles , connective tissue and vascularization .
	manualset3
202078	2	417475	7	NULL	NULL	0	NULL	internal urethral structures	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	What is said so far must not exclude the importance of recognizing the role of the internal urethral structures to maintain continence , in particular the quality of urethral muscles , connective tissue and vascularization .
	manualset3
202079	3	417475	7	NULL	NULL	0	NULL	continence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	What is said so far must not exclude the importance of recognizing the role of the internal urethral structures to maintain continence , in particular the quality of urethral muscles , connective tissue and vascularization .
	manualset3
202080	4	417475	7	NULL	NULL	0	NULL	quality	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	What is said so far must not exclude the importance of recognizing the role of the internal urethral structures to maintain continence , in particular the quality of urethral muscles , connective tissue and vascularization .
	manualset3
202081	5	417475	7	NULL	NULL	0	NULL	 urethral muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	What is said so far must not exclude the importance of recognizing the role of the internal urethral structures to maintain continence , in particular the quality of urethral muscles , connective tissue and vascularization .
	manualset3
202082	6	417475	7	NULL	NULL	0	NULL	connective tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	What is said so far must not exclude the importance of recognizing the role of the internal urethral structures to maintain continence , in particular the quality of urethral muscles , connective tissue and vascularization .
	manualset3
202083	7	417475	7	NULL	NULL	0	NULL	 vascularization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	What is said so far must not exclude the importance of recognizing the role of the internal urethral structures to maintain continence , in particular the quality of urethral muscles , connective tissue and vascularization .
	manualset3
202085	1	417476	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	What is the best for patient ?
	manualset3
202086	1	417477	7	NULL	NULL	0	NULL	evidence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	What is the evidence behind the evidence-base ?
	manualset3
202087	2	417477	7	NULL	NULL	0	NULL	evidence-base	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	What is the evidence behind the evidence-base ?
	manualset3
202088	1	417478	7	NULL	NULL	0	NULL	history	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	What is the history of bioethics ?
	manualset3
202089	2	417478	7	NULL	NULL	0	NULL	bioethics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	What is the history of bioethics ?
	manualset3
202090	1	417479	7	NULL	NULL	0	NULL	 real toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	What is their real toxicity ? ) .
	manualset3
202091	1	417480	7	NULL	NULL	0	NULL	melody 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	What makes a melody : The perceptual singularity of pitch sequences .
	manualset3
202092	2	417480	7	NULL	NULL	0	NULL	perceptual singularity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	What makes a melody : The perceptual singularity of pitch sequences .
	manualset3
202093	3	417480	7	NULL	NULL	0	NULL	pitch sequences	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	What makes a melody : The perceptual singularity of pitch sequences .
	manualset3
202094	1	417481	7	NULL	NULL	0	NULL	lungs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	All lungs had centrilobular emphysema .
	manualset3
202095	2	417481	7	NULL	NULL	0	NULL	centrilobular emphysema	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All lungs had centrilobular emphysema .
	manualset3
202096	1	417482	7	NULL	NULL	0	NULL	 man 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	What man can do technologically to restore his environment .
	manualset3
202097	2	417482	7	NULL	NULL	0	NULL	environment 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	What man can do technologically to restore his environment .
	manualset3
202098	1	417483	7	NULL	NULL	NULL	NULL	men 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	What men say about surviving prostate cancer : complexities represented in a decade of comments .
	manualset3
202099	2	417483	7	NULL	NULL	0	NULL	prostate cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	What men say about surviving prostate cancer : complexities represented in a decade of comments .
	manualset3
202100	3	417483	7	NULL	NULL	0	NULL	complexities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	What men say about surviving prostate cancer : complexities represented in a decade of comments .
	manualset3
202101	4	417483	7	NULL	NULL	0	NULL	decade	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	What men say about surviving prostate cancer : complexities represented in a decade of comments .
	manualset3
202102	5	417483	7	NULL	NULL	0	NULL	comments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	What men say about surviving prostate cancer : complexities represented in a decade of comments .
	manualset3
202103	1	417484	7	NULL	NULL	0	NULL	situation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	What of the situation in low income countries where the highest proportion of the tuberculosis patients live at the present time ?
	manualset3
202104	2	417484	7	NULL	NULL	0	NULL	 low income countries	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	What of the situation in low income countries where the highest proportion of the tuberculosis patients live at the present time ?
	manualset3
202105	3	417484	7	NULL	NULL	0	NULL	highest proportion	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	What of the situation in low income countries where the highest proportion of the tuberculosis patients live at the present time ?
	manualset3
202106	4	417484	7	NULL	NULL	0	NULL	tuberculosis patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	What of the situation in low income countries where the highest proportion of the tuberculosis patients live at the present time ?
	manualset3
202107	5	417484	7	NULL	NULL	NULL	NULL	present time	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	What of the situation in low income countries where the highest proportion of the tuberculosis patients live at the present time ?
	manualset3
202108	1	417485	7	NULL	NULL	0	NULL	weight regain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	What predicts weight regain in a group of successful weight losers ? .
	manualset3
202109	2	417485	7	NULL	NULL	0	NULL	group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	What predicts weight regain in a group of successful weight losers ? .
	manualset3
202110	3	417485	7	NULL	NULL	0	NULL	 weight losers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	What predicts weight regain in a group of successful weight losers ? .
	manualset3
202111	1	417486	7	NULL	NULL	0	NULL	principles	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	What principles guide research with human participants ?
	manualset3
202112	2	417486	7	NULL	NULL	0	NULL	 research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	What principles guide research with human participants ?
	manualset3
202113	3	417486	7	NULL	NULL	0	NULL	human participants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	What principles guide research with human participants ?
	manualset3
202114	1	417487	7	NULL	NULL	0	NULL	spouse caregivers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	What spouse caregivers know about communication in Alzheimer 's disease : development of the AD Communication Knowledge Test .
	manualset3
202115	2	417487	7	NULL	NULL	0	NULL	communication	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	What spouse caregivers know about communication in Alzheimer 's disease : development of the AD Communication Knowledge Test .
	manualset3
202116	3	417487	7	NULL	NULL	0	NULL	Alzheimer 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	What spouse caregivers know about communication in Alzheimer 's disease : development of the AD Communication Knowledge Test .
	manualset3
202117	4	417487	7	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	What spouse caregivers know about communication in Alzheimer 's disease : development of the AD Communication Knowledge Test .
	manualset3
202118	5	417487	7	NULL	NULL	0	NULL	AD Communication Knowledge Test	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	What spouse caregivers know about communication in Alzheimer 's disease : development of the AD Communication Knowledge Test .
	manualset3
202119	1	417488	7	NULL	NULL	NULL	NULL	GI approach	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	What will be our GI approach to a child with FTT syndrome ?
	manualset3
202120	2	417488	7	NULL	NULL	0	NULL	child 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	What will be our GI approach to a child with FTT syndrome ?
	manualset3
202121	3	417488	7	NULL	NULL	NULL	NULL	 FTT syndrome	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	What will be our GI approach to a child with FTT syndrome ?
	manualset3
202122	1	417489	7	NULL	NULL	0	NULL	mechanism 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Whatever is the mechanism of the disease , the characterization of large numbers of renin-containing cells in the affected kidney support a role for the renin-angiotensin system stimulation in this form of hypertension .
	manualset3
202123	2	417489	7	NULL	NULL	0	NULL	disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Whatever is the mechanism of the disease , the characterization of large numbers of renin-containing cells in the affected kidney support a role for the renin-angiotensin system stimulation in this form of hypertension .
	manualset3
202124	3	417489	7	NULL	NULL	NULL	NULL	characterization	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Whatever is the mechanism of the disease , the characterization of large numbers of renin-containing cells in the affected kidney support a role for the renin-angiotensin system stimulation in this form of hypertension .
	manualset3
202125	4	417489	7	NULL	NULL	0	NULL	large numbers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Whatever is the mechanism of the disease , the characterization of large numbers of renin-containing cells in the affected kidney support a role for the renin-angiotensin system stimulation in this form of hypertension .
	manualset3
202126	5	417489	7	NULL	NULL	0	NULL	renin-containing cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Whatever is the mechanism of the disease , the characterization of large numbers of renin-containing cells in the affected kidney support a role for the renin-angiotensin system stimulation in this form of hypertension .
	manualset3
202127	6	417489	7	NULL	NULL	0	NULL	affected kidney	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Whatever is the mechanism of the disease , the characterization of large numbers of renin-containing cells in the affected kidney support a role for the renin-angiotensin system stimulation in this form of hypertension .
	manualset3
202128	7	417489	7	NULL	NULL	0	NULL	 role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Whatever is the mechanism of the disease , the characterization of large numbers of renin-containing cells in the affected kidney support a role for the renin-angiotensin system stimulation in this form of hypertension .
	manualset3
202129	8	417489	7	NULL	NULL	0	NULL	renin-angiotensin system stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Whatever is the mechanism of the disease , the characterization of large numbers of renin-containing cells in the affected kidney support a role for the renin-angiotensin system stimulation in this form of hypertension .
	manualset3
202130	9	417489	7	NULL	NULL	0	NULL	hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Whatever is the mechanism of the disease , the characterization of large numbers of renin-containing cells in the affected kidney support a role for the renin-angiotensin system stimulation in this form of hypertension .
	manualset3
202131	1	417490	7	NULL	NULL	0	NULL	72 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When 72 % of the carboxyl groups in gamma-PGA were sulfonated ( gamma-PGA-S72 ) , cell numbers reached a maximum .
	manualset3
202132	2	417490	7	NULL	NULL	0	NULL	carboxyl groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When 72 % of the carboxyl groups in gamma-PGA were sulfonated ( gamma-PGA-S72 ) , cell numbers reached a maximum .
	manualset3
202133	3	417490	7	NULL	NULL	0	NULL	gamma-PGA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When 72 % of the carboxyl groups in gamma-PGA were sulfonated ( gamma-PGA-S72 ) , cell numbers reached a maximum .
	manualset3
202134	4	417490	7	NULL	NULL	0	NULL	gamma-PGA-S72	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When 72 % of the carboxyl groups in gamma-PGA were sulfonated ( gamma-PGA-S72 ) , cell numbers reached a maximum .
	manualset3
202135	5	417490	7	NULL	NULL	0	NULL	cell numbers	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	When 72 % of the carboxyl groups in gamma-PGA were sulfonated ( gamma-PGA-S72 ) , cell numbers reached a maximum .
	manualset3
202136	1	417491	7	NULL	NULL	0	NULL	BSA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When BSA and poly ( L-proline ) form films on quartz , their secondary structures change significantly : 13 % for BSA and 32 % for poly ( L-proline ) .
	manualset3
202137	2	417491	7	NULL	NULL	NULL	NULL	poly ( L-proline )	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When BSA and poly ( L-proline ) form films on quartz , their secondary structures change significantly : 13 % for BSA and 32 % for poly ( L-proline ) .
	manualset3
202138	3	417491	7	NULL	NULL	0	NULL	films 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When BSA and poly ( L-proline ) form films on quartz , their secondary structures change significantly : 13 % for BSA and 32 % for poly ( L-proline ) .
	manualset3
202139	4	417491	7	NULL	NULL	0	NULL	quartz	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When BSA and poly ( L-proline ) form films on quartz , their secondary structures change significantly : 13 % for BSA and 32 % for poly ( L-proline ) .
	manualset3
202140	5	417491	7	NULL	NULL	NULL	NULL	secondary structures 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When BSA and poly ( L-proline ) form films on quartz , their secondary structures change significantly : 13 % for BSA and 32 % for poly ( L-proline ) .
	manualset3
202141	6	417491	7	NULL	NULL	0	NULL	13 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When BSA and poly ( L-proline ) form films on quartz , their secondary structures change significantly : 13 % for BSA and 32 % for poly ( L-proline ) .
	manualset3
202142	7	417491	7	NULL	NULL	0	NULL	BSA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When BSA and poly ( L-proline ) form films on quartz , their secondary structures change significantly : 13 % for BSA and 32 % for poly ( L-proline ) .
	manualset3
202143	8	417491	7	NULL	NULL	0	NULL	 32 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When BSA and poly ( L-proline ) form films on quartz , their secondary structures change significantly : 13 % for BSA and 32 % for poly ( L-proline ) .
	manualset3
202144	9	417491	7	NULL	NULL	0	NULL	poly ( L-proline )	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	When BSA and poly ( L-proline ) form films on quartz , their secondary structures change significantly : 13 % for BSA and 32 % for poly ( L-proline ) .
	manualset3
202145	1	417492	7	NULL	NULL	0	NULL	C57BL/6J males	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When C57BL/6J males were exposed to a 50 Hz , 45 kV/m electric field for 30 min per day for 11 days and placed in a cage with a superovulated female of the same strain , the successful copulation rates of males was significantly improved compared with unexposed males ( P & lt ; 0.05 ) .
	manualset3
202146	2	417492	7	NULL	NULL	0	NULL	 50 Hz	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When C57BL/6J males were exposed to a 50 Hz , 45 kV/m electric field for 30 min per day for 11 days and placed in a cage with a superovulated female of the same strain , the successful copulation rates of males was significantly improved compared with unexposed males ( P & lt ; 0.05 ) .
	manualset3
202147	3	417492	7	NULL	NULL	0	NULL	 45 kV/m electric field 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When C57BL/6J males were exposed to a 50 Hz , 45 kV/m electric field for 30 min per day for 11 days and placed in a cage with a superovulated female of the same strain , the successful copulation rates of males was significantly improved compared with unexposed males ( P & lt ; 0.05 ) .
	manualset3
202148	4	417492	7	NULL	NULL	0	NULL	30 min per day	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	When C57BL/6J males were exposed to a 50 Hz , 45 kV/m electric field for 30 min per day for 11 days and placed in a cage with a superovulated female of the same strain , the successful copulation rates of males was significantly improved compared with unexposed males ( P & lt ; 0.05 ) .
	manualset3
202149	5	417492	7	NULL	NULL	0	NULL	11 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	When C57BL/6J males were exposed to a 50 Hz , 45 kV/m electric field for 30 min per day for 11 days and placed in a cage with a superovulated female of the same strain , the successful copulation rates of males was significantly improved compared with unexposed males ( P & lt ; 0.05 ) .
	manualset3
202150	6	417492	7	NULL	NULL	0	NULL	 cage	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	When C57BL/6J males were exposed to a 50 Hz , 45 kV/m electric field for 30 min per day for 11 days and placed in a cage with a superovulated female of the same strain , the successful copulation rates of males was significantly improved compared with unexposed males ( P & lt ; 0.05 ) .
	manualset3
202151	7	417492	7	NULL	NULL	0	NULL	superovulated female	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When C57BL/6J males were exposed to a 50 Hz , 45 kV/m electric field for 30 min per day for 11 days and placed in a cage with a superovulated female of the same strain , the successful copulation rates of males was significantly improved compared with unexposed males ( P & lt ; 0.05 ) .
	manualset3
202152	8	417492	7	NULL	NULL	0	NULL	strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When C57BL/6J males were exposed to a 50 Hz , 45 kV/m electric field for 30 min per day for 11 days and placed in a cage with a superovulated female of the same strain , the successful copulation rates of males was significantly improved compared with unexposed males ( P & lt ; 0.05 ) .
	manualset3
202153	9	417492	7	NULL	NULL	0	NULL	copulation rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When C57BL/6J males were exposed to a 50 Hz , 45 kV/m electric field for 30 min per day for 11 days and placed in a cage with a superovulated female of the same strain , the successful copulation rates of males was significantly improved compared with unexposed males ( P & lt ; 0.05 ) .
	manualset3
202154	10	417492	7	NULL	NULL	0	NULL	males	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When C57BL/6J males were exposed to a 50 Hz , 45 kV/m electric field for 30 min per day for 11 days and placed in a cage with a superovulated female of the same strain , the successful copulation rates of males was significantly improved compared with unexposed males ( P & lt ; 0.05 ) .
	manualset3
202155	11	417492	7	NULL	NULL	NULL	NULL	unexposed males	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When C57BL/6J males were exposed to a 50 Hz , 45 kV/m electric field for 30 min per day for 11 days and placed in a cage with a superovulated female of the same strain , the successful copulation rates of males was significantly improved compared with unexposed males ( P & lt ; 0.05 ) .
	manualset3
202156	12	417492	7	NULL	NULL	0	NULL	P & lt ; 0.05 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When C57BL/6J males were exposed to a 50 Hz , 45 kV/m electric field for 30 min per day for 11 days and placed in a cage with a superovulated female of the same strain , the successful copulation rates of males was significantly improved compared with unexposed males ( P & lt ; 0.05 ) .
	manualset3
202157	1	417493	7	NULL	NULL	0	NULL	COS-1 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	When COS-1 cells were transfected with type II receptor cDNAs , GDF-5 bound to ActR-II , ActR-IIB , and BMPR-II but not to transforming growth factor-beta type II receptor .
	manualset3
202158	2	417493	7	NULL	NULL	0	NULL	 type II receptor cDNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	When COS-1 cells were transfected with type II receptor cDNAs , GDF-5 bound to ActR-II , ActR-IIB , and BMPR-II but not to transforming growth factor-beta type II receptor .
	manualset3
202159	3	417493	7	NULL	NULL	0	NULL	GDF-5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When COS-1 cells were transfected with type II receptor cDNAs , GDF-5 bound to ActR-II , ActR-IIB , and BMPR-II but not to transforming growth factor-beta type II receptor .
	manualset3
202160	4	417493	7	NULL	NULL	0	NULL	ActR-II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When COS-1 cells were transfected with type II receptor cDNAs , GDF-5 bound to ActR-II , ActR-IIB , and BMPR-II but not to transforming growth factor-beta type II receptor .
	manualset3
202161	5	417493	7	NULL	NULL	0	NULL	ActR-IIB	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When COS-1 cells were transfected with type II receptor cDNAs , GDF-5 bound to ActR-II , ActR-IIB , and BMPR-II but not to transforming growth factor-beta type II receptor .
	manualset3
202162	6	417493	7	NULL	NULL	0	NULL	BMPR-II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When COS-1 cells were transfected with type II receptor cDNAs , GDF-5 bound to ActR-II , ActR-IIB , and BMPR-II but not to transforming growth factor-beta type II receptor .
	manualset3
202163	7	417493	7	NULL	NULL	0	NULL	transforming growth factor-beta type II receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When COS-1 cells were transfected with type II receptor cDNAs , GDF-5 bound to ActR-II , ActR-IIB , and BMPR-II but not to transforming growth factor-beta type II receptor .
	manualset3
202164	1	417494	7	NULL	NULL	0	NULL	CV-1 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	When CV-1 cells were transfected with human glucocorticoid receptor ( hGR ) rather than hAR , PME failed to significantly induce MMTV-luciferase expression .
	manualset3
202165	2	417494	7	NULL	NULL	0	NULL	human glucocorticoid receptor ( hGR )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When CV-1 cells were transfected with human glucocorticoid receptor ( hGR ) rather than hAR , PME failed to significantly induce MMTV-luciferase expression .
	manualset3
202166	3	417494	7	NULL	NULL	0	NULL	hAR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When CV-1 cells were transfected with human glucocorticoid receptor ( hGR ) rather than hAR , PME failed to significantly induce MMTV-luciferase expression .
	manualset3
202167	4	417494	7	NULL	NULL	0	NULL	PME	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When CV-1 cells were transfected with human glucocorticoid receptor ( hGR ) rather than hAR , PME failed to significantly induce MMTV-luciferase expression .
	manualset3
202168	5	417494	7	NULL	NULL	0	NULL	MMTV-luciferase expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When CV-1 cells were transfected with human glucocorticoid receptor ( hGR ) rather than hAR , PME failed to significantly induce MMTV-luciferase expression .
	manualset3
202169	1	417495	7	NULL	NULL	0	NULL	Gly2-Lys-Gly3	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	When Gly2-Lys-Gly3 and Tos-Arg-OMe were used as substrates , the values of I50 for the peptide Ia were calculated to be 3.6 micron and 40 micron , respectively .
	manualset3
202170	2	417495	7	NULL	NULL	0	NULL	Tos-Arg-OMe	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When Gly2-Lys-Gly3 and Tos-Arg-OMe were used as substrates , the values of I50 for the peptide Ia were calculated to be 3.6 micron and 40 micron , respectively .
	manualset3
202171	3	417495	7	NULL	NULL	0	NULL	substrates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When Gly2-Lys-Gly3 and Tos-Arg-OMe were used as substrates , the values of I50 for the peptide Ia were calculated to be 3.6 micron and 40 micron , respectively .
	manualset3
202172	4	417495	7	NULL	NULL	0	NULL	values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When Gly2-Lys-Gly3 and Tos-Arg-OMe were used as substrates , the values of I50 for the peptide Ia were calculated to be 3.6 micron and 40 micron , respectively .
	manualset3
202173	5	417495	7	NULL	NULL	0	NULL	I50	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When Gly2-Lys-Gly3 and Tos-Arg-OMe were used as substrates , the values of I50 for the peptide Ia were calculated to be 3.6 micron and 40 micron , respectively .
	manualset3
202174	6	417495	7	NULL	NULL	0	NULL	peptide Ia 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	When Gly2-Lys-Gly3 and Tos-Arg-OMe were used as substrates , the values of I50 for the peptide Ia were calculated to be 3.6 micron and 40 micron , respectively .
	manualset3
202175	7	417495	7	NULL	NULL	0	NULL	 3.6 micron	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	When Gly2-Lys-Gly3 and Tos-Arg-OMe were used as substrates , the values of I50 for the peptide Ia were calculated to be 3.6 micron and 40 micron , respectively .
	manualset3
202176	8	417495	7	NULL	NULL	0	NULL	40 micron	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	When Gly2-Lys-Gly3 and Tos-Arg-OMe were used as substrates , the values of I50 for the peptide Ia were calculated to be 3.6 micron and 40 micron , respectively .
	manualset3
202177	1	417496	7	NULL	NULL	0	NULL	HSL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When HSL was blocked by compound 76-0079 , free fatty acid release was still induced by resveratrol .
	manualset3
202178	2	417496	7	NULL	NULL	0	NULL	compound 76-0079	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When HSL was blocked by compound 76-0079 , free fatty acid release was still induced by resveratrol .
	manualset3
202179	3	417496	7	NULL	NULL	0	NULL	free fatty acid release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When HSL was blocked by compound 76-0079 , free fatty acid release was still induced by resveratrol .
	manualset3
202180	4	417496	7	NULL	NULL	0	NULL	 resveratrol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When HSL was blocked by compound 76-0079 , free fatty acid release was still induced by resveratrol .
	manualset3
202181	1	417497	7	NULL	NULL	0	NULL	HVc explants	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When HVc explants derived from adult zebra finches were maintained in low-serum medium , in vitro neurogenesis could be demonstrated by 3H-thymidine uptake as long as 5 days after explantation .
	manualset3
202182	2	417497	7	NULL	NULL	0	NULL	adult zebra finches	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When HVc explants derived from adult zebra finches were maintained in low-serum medium , in vitro neurogenesis could be demonstrated by 3H-thymidine uptake as long as 5 days after explantation .
	manualset3
202183	3	417497	7	NULL	NULL	0	NULL	low-serum medium	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	When HVc explants derived from adult zebra finches were maintained in low-serum medium , in vitro neurogenesis could be demonstrated by 3H-thymidine uptake as long as 5 days after explantation .
	manualset3
202184	4	417497	7	NULL	NULL	0	NULL	in vitro neurogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When HVc explants derived from adult zebra finches were maintained in low-serum medium , in vitro neurogenesis could be demonstrated by 3H-thymidine uptake as long as 5 days after explantation .
	manualset3
202185	5	417497	7	NULL	NULL	0	NULL	3H-thymidine uptake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When HVc explants derived from adult zebra finches were maintained in low-serum medium , in vitro neurogenesis could be demonstrated by 3H-thymidine uptake as long as 5 days after explantation .
	manualset3
202186	6	417497	7	NULL	NULL	0	NULL	5 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	When HVc explants derived from adult zebra finches were maintained in low-serum medium , in vitro neurogenesis could be demonstrated by 3H-thymidine uptake as long as 5 days after explantation .
	manualset3
202187	7	417497	7	NULL	NULL	0	NULL	explantation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When HVc explants derived from adult zebra finches were maintained in low-serum medium , in vitro neurogenesis could be demonstrated by 3H-thymidine uptake as long as 5 days after explantation .
	manualset3
202188	1	417498	7	NULL	NULL	0	NULL	IC2 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	When IC2 cells were cultured with saturating concentrations of IL-3 , GM-CSF or a combination of both , the doubling time was 25 + / - 1 h , whereas it decreased to 17 + / - 1 h when IL-4 was further added to the cultures .
	manualset3
202189	2	417498	7	NULL	NULL	0	NULL	saturating concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When IC2 cells were cultured with saturating concentrations of IL-3 , GM-CSF or a combination of both , the doubling time was 25 + / - 1 h , whereas it decreased to 17 + / - 1 h when IL-4 was further added to the cultures .
	manualset3
202190	3	417498	7	NULL	NULL	0	NULL	IL-3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When IC2 cells were cultured with saturating concentrations of IL-3 , GM-CSF or a combination of both , the doubling time was 25 + / - 1 h , whereas it decreased to 17 + / - 1 h when IL-4 was further added to the cultures .
	manualset3
202191	4	417498	7	NULL	NULL	0	NULL	GM-CSF	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When IC2 cells were cultured with saturating concentrations of IL-3 , GM-CSF or a combination of both , the doubling time was 25 + / - 1 h , whereas it decreased to 17 + / - 1 h when IL-4 was further added to the cultures .
	manualset3
202192	5	417498	7	NULL	NULL	0	NULL	 combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When IC2 cells were cultured with saturating concentrations of IL-3 , GM-CSF or a combination of both , the doubling time was 25 + / - 1 h , whereas it decreased to 17 + / - 1 h when IL-4 was further added to the cultures .
	manualset3
202193	6	417498	7	NULL	NULL	0	NULL	doubling time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	When IC2 cells were cultured with saturating concentrations of IL-3 , GM-CSF or a combination of both , the doubling time was 25 + / - 1 h , whereas it decreased to 17 + / - 1 h when IL-4 was further added to the cultures .
	manualset3
202194	7	417498	7	NULL	NULL	0	NULL	25 + / - 1 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	When IC2 cells were cultured with saturating concentrations of IL-3 , GM-CSF or a combination of both , the doubling time was 25 + / - 1 h , whereas it decreased to 17 + / - 1 h when IL-4 was further added to the cultures .
	manualset3
202195	8	417498	7	NULL	NULL	0	NULL	17 + / - 1 h 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	When IC2 cells were cultured with saturating concentrations of IL-3 , GM-CSF or a combination of both , the doubling time was 25 + / - 1 h , whereas it decreased to 17 + / - 1 h when IL-4 was further added to the cultures .
	manualset3
202196	9	417498	7	NULL	NULL	0	NULL	IL-4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When IC2 cells were cultured with saturating concentrations of IL-3 , GM-CSF or a combination of both , the doubling time was 25 + / - 1 h , whereas it decreased to 17 + / - 1 h when IL-4 was further added to the cultures .
	manualset3
202197	10	417498	7	NULL	NULL	0	NULL	cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	When IC2 cells were cultured with saturating concentrations of IL-3 , GM-CSF or a combination of both , the doubling time was 25 + / - 1 h , whereas it decreased to 17 + / - 1 h when IL-4 was further added to the cultures .
	manualset3
202198	1	417499	7	NULL	NULL	0	NULL	NADPH-fortified microsomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	When NADPH-fortified microsomes were incubated with N-nitroso-N-methylvinylamine , HCHO was formed , and when DNA was included in incubations , 1 , N6-epsilon-dAdo and N7-methylGua were isolated from DNA .
	manualset3
202199	2	417499	7	NULL	NULL	0	NULL	N-nitroso-N-methylvinylamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When NADPH-fortified microsomes were incubated with N-nitroso-N-methylvinylamine , HCHO was formed , and when DNA was included in incubations , 1 , N6-epsilon-dAdo and N7-methylGua were isolated from DNA .
	manualset3
202200	3	417499	7	NULL	NULL	0	NULL	HCHO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When NADPH-fortified microsomes were incubated with N-nitroso-N-methylvinylamine , HCHO was formed , and when DNA was included in incubations , 1 , N6-epsilon-dAdo and N7-methylGua were isolated from DNA .
	manualset3
202201	4	417499	7	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	When NADPH-fortified microsomes were incubated with N-nitroso-N-methylvinylamine , HCHO was formed , and when DNA was included in incubations , 1 , N6-epsilon-dAdo and N7-methylGua were isolated from DNA .
	manualset3
202202	5	417499	7	NULL	NULL	0	NULL	 incubations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	When NADPH-fortified microsomes were incubated with N-nitroso-N-methylvinylamine , HCHO was formed , and when DNA was included in incubations , 1 , N6-epsilon-dAdo and N7-methylGua were isolated from DNA .
	manualset3
202203	6	417499	7	NULL	NULL	0	NULL	 1 , N6-epsilon-dAdo	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When NADPH-fortified microsomes were incubated with N-nitroso-N-methylvinylamine , HCHO was formed , and when DNA was included in incubations , 1 , N6-epsilon-dAdo and N7-methylGua were isolated from DNA .
	manualset3
202204	7	417499	7	NULL	NULL	0	NULL	N7-methylGua	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When NADPH-fortified microsomes were incubated with N-nitroso-N-methylvinylamine , HCHO was formed , and when DNA was included in incubations , 1 , N6-epsilon-dAdo and N7-methylGua were isolated from DNA .
	manualset3
202205	8	417499	7	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	When NADPH-fortified microsomes were incubated with N-nitroso-N-methylvinylamine , HCHO was formed , and when DNA was included in incubations , 1 , N6-epsilon-dAdo and N7-methylGua were isolated from DNA .
	manualset3
202206	1	417500	7	NULL	NULL	0	NULL	NTERA-2 cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	When NTERA-2 cells were induced to differentiate by culturing in the presence of 10 ( -5 ) M retinoic acid , a remarkable shift of cellular glycolipids from globo-series to lacto - and ganglio-series was observed : Globo-series structures declined , particularly during the period 7-20 days after first exposure to retinoic acid , while lacto-series structures , including fucosyl alpha 1 -- 3 type 2 chain ( Lex ) and sialosyl type 2 chain , and ganglio-series structures , including GM3 , GD3 , 9-O-acetyl-GD3 , GM2 , GD2 , and GT3 , increased .
	manualset3
202207	2	417500	7	NULL	NULL	0	NULL	culturing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	When NTERA-2 cells were induced to differentiate by culturing in the presence of 10 ( -5 ) M retinoic acid , a remarkable shift of cellular glycolipids from globo-series to lacto - and ganglio-series was observed : Globo-series structures declined , particularly during the period 7-20 days after first exposure to retinoic acid , while lacto-series structures , including fucosyl alpha 1 -- 3 type 2 chain ( Lex ) and sialosyl type 2 chain , and ganglio-series structures , including GM3 , GD3 , 9-O-acetyl-GD3 , GM2 , GD2 , and GT3 , increased .
	manualset3
202208	3	417500	7	NULL	NULL	0	NULL	10 ( -5 ) M 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	When NTERA-2 cells were induced to differentiate by culturing in the presence of 10 ( -5 ) M retinoic acid , a remarkable shift of cellular glycolipids from globo-series to lacto - and ganglio-series was observed : Globo-series structures declined , particularly during the period 7-20 days after first exposure to retinoic acid , while lacto-series structures , including fucosyl alpha 1 -- 3 type 2 chain ( Lex ) and sialosyl type 2 chain , and ganglio-series structures , including GM3 , GD3 , 9-O-acetyl-GD3 , GM2 , GD2 , and GT3 , increased .
	manualset3
202209	4	417500	7	NULL	NULL	0	NULL	 retinoic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When NTERA-2 cells were induced to differentiate by culturing in the presence of 10 ( -5 ) M retinoic acid , a remarkable shift of cellular glycolipids from globo-series to lacto - and ganglio-series was observed : Globo-series structures declined , particularly during the period 7-20 days after first exposure to retinoic acid , while lacto-series structures , including fucosyl alpha 1 -- 3 type 2 chain ( Lex ) and sialosyl type 2 chain , and ganglio-series structures , including GM3 , GD3 , 9-O-acetyl-GD3 , GM2 , GD2 , and GT3 , increased .
	manualset3
202210	5	417500	7	NULL	NULL	0	NULL	remarkable shift	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When NTERA-2 cells were induced to differentiate by culturing in the presence of 10 ( -5 ) M retinoic acid , a remarkable shift of cellular glycolipids from globo-series to lacto - and ganglio-series was observed : Globo-series structures declined , particularly during the period 7-20 days after first exposure to retinoic acid , while lacto-series structures , including fucosyl alpha 1 -- 3 type 2 chain ( Lex ) and sialosyl type 2 chain , and ganglio-series structures , including GM3 , GD3 , 9-O-acetyl-GD3 , GM2 , GD2 , and GT3 , increased .
	manualset3
202211	6	417500	7	NULL	NULL	0	NULL	cellular glycolipids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When NTERA-2 cells were induced to differentiate by culturing in the presence of 10 ( -5 ) M retinoic acid , a remarkable shift of cellular glycolipids from globo-series to lacto - and ganglio-series was observed : Globo-series structures declined , particularly during the period 7-20 days after first exposure to retinoic acid , while lacto-series structures , including fucosyl alpha 1 -- 3 type 2 chain ( Lex ) and sialosyl type 2 chain , and ganglio-series structures , including GM3 , GD3 , 9-O-acetyl-GD3 , GM2 , GD2 , and GT3 , increased .
	manualset3
202212	7	417500	7	NULL	NULL	NULL	NULL	globo-series 	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When NTERA-2 cells were induced to differentiate by culturing in the presence of 10 ( -5 ) M retinoic acid , a remarkable shift of cellular glycolipids from globo-series to lacto - and ganglio-series was observed : Globo-series structures declined , particularly during the period 7-20 days after first exposure to retinoic acid , while lacto-series structures , including fucosyl alpha 1 -- 3 type 2 chain ( Lex ) and sialosyl type 2 chain , and ganglio-series structures , including GM3 , GD3 , 9-O-acetyl-GD3 , GM2 , GD2 , and GT3 , increased .
	manualset3
202213	8	417500	7	NULL	NULL	NULL	NULL	ganglio-series	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When NTERA-2 cells were induced to differentiate by culturing in the presence of 10 ( -5 ) M retinoic acid , a remarkable shift of cellular glycolipids from globo-series to lacto - and ganglio-series was observed : Globo-series structures declined , particularly during the period 7-20 days after first exposure to retinoic acid , while lacto-series structures , including fucosyl alpha 1 -- 3 type 2 chain ( Lex ) and sialosyl type 2 chain , and ganglio-series structures , including GM3 , GD3 , 9-O-acetyl-GD3 , GM2 , GD2 , and GT3 , increased .
	manualset3
202214	9	417500	7	NULL	NULL	0	NULL	Globo-series structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When NTERA-2 cells were induced to differentiate by culturing in the presence of 10 ( -5 ) M retinoic acid , a remarkable shift of cellular glycolipids from globo-series to lacto - and ganglio-series was observed : Globo-series structures declined , particularly during the period 7-20 days after first exposure to retinoic acid , while lacto-series structures , including fucosyl alpha 1 -- 3 type 2 chain ( Lex ) and sialosyl type 2 chain , and ganglio-series structures , including GM3 , GD3 , 9-O-acetyl-GD3 , GM2 , GD2 , and GT3 , increased .
	manualset3
202215	10	417500	7	NULL	NULL	0	NULL	 period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	When NTERA-2 cells were induced to differentiate by culturing in the presence of 10 ( -5 ) M retinoic acid , a remarkable shift of cellular glycolipids from globo-series to lacto - and ganglio-series was observed : Globo-series structures declined , particularly during the period 7-20 days after first exposure to retinoic acid , while lacto-series structures , including fucosyl alpha 1 -- 3 type 2 chain ( Lex ) and sialosyl type 2 chain , and ganglio-series structures , including GM3 , GD3 , 9-O-acetyl-GD3 , GM2 , GD2 , and GT3 , increased .
	manualset3
202216	11	417500	7	NULL	NULL	0	NULL	7-20 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	When NTERA-2 cells were induced to differentiate by culturing in the presence of 10 ( -5 ) M retinoic acid , a remarkable shift of cellular glycolipids from globo-series to lacto - and ganglio-series was observed : Globo-series structures declined , particularly during the period 7-20 days after first exposure to retinoic acid , while lacto-series structures , including fucosyl alpha 1 -- 3 type 2 chain ( Lex ) and sialosyl type 2 chain , and ganglio-series structures , including GM3 , GD3 , 9-O-acetyl-GD3 , GM2 , GD2 , and GT3 , increased .
	manualset3
202217	12	417500	7	NULL	NULL	0	NULL	 first exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When NTERA-2 cells were induced to differentiate by culturing in the presence of 10 ( -5 ) M retinoic acid , a remarkable shift of cellular glycolipids from globo-series to lacto - and ganglio-series was observed : Globo-series structures declined , particularly during the period 7-20 days after first exposure to retinoic acid , while lacto-series structures , including fucosyl alpha 1 -- 3 type 2 chain ( Lex ) and sialosyl type 2 chain , and ganglio-series structures , including GM3 , GD3 , 9-O-acetyl-GD3 , GM2 , GD2 , and GT3 , increased .
	manualset3
202218	13	417500	7	NULL	NULL	0	NULL	retinoic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When NTERA-2 cells were induced to differentiate by culturing in the presence of 10 ( -5 ) M retinoic acid , a remarkable shift of cellular glycolipids from globo-series to lacto - and ganglio-series was observed : Globo-series structures declined , particularly during the period 7-20 days after first exposure to retinoic acid , while lacto-series structures , including fucosyl alpha 1 -- 3 type 2 chain ( Lex ) and sialosyl type 2 chain , and ganglio-series structures , including GM3 , GD3 , 9-O-acetyl-GD3 , GM2 , GD2 , and GT3 , increased .
	manualset3
202219	14	417500	7	NULL	NULL	0	NULL	lacto-series structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When NTERA-2 cells were induced to differentiate by culturing in the presence of 10 ( -5 ) M retinoic acid , a remarkable shift of cellular glycolipids from globo-series to lacto - and ganglio-series was observed : Globo-series structures declined , particularly during the period 7-20 days after first exposure to retinoic acid , while lacto-series structures , including fucosyl alpha 1 -- 3 type 2 chain ( Lex ) and sialosyl type 2 chain , and ganglio-series structures , including GM3 , GD3 , 9-O-acetyl-GD3 , GM2 , GD2 , and GT3 , increased .
	manualset3
202220	15	417500	7	NULL	NULL	0	NULL	fucosyl alpha 1 -- 3 type 2 chain ( Lex ) 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When NTERA-2 cells were induced to differentiate by culturing in the presence of 10 ( -5 ) M retinoic acid , a remarkable shift of cellular glycolipids from globo-series to lacto - and ganglio-series was observed : Globo-series structures declined , particularly during the period 7-20 days after first exposure to retinoic acid , while lacto-series structures , including fucosyl alpha 1 -- 3 type 2 chain ( Lex ) and sialosyl type 2 chain , and ganglio-series structures , including GM3 , GD3 , 9-O-acetyl-GD3 , GM2 , GD2 , and GT3 , increased .
	manualset3
202221	16	417500	7	NULL	NULL	0	NULL	sialosyl type 2 chain 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When NTERA-2 cells were induced to differentiate by culturing in the presence of 10 ( -5 ) M retinoic acid , a remarkable shift of cellular glycolipids from globo-series to lacto - and ganglio-series was observed : Globo-series structures declined , particularly during the period 7-20 days after first exposure to retinoic acid , while lacto-series structures , including fucosyl alpha 1 -- 3 type 2 chain ( Lex ) and sialosyl type 2 chain , and ganglio-series structures , including GM3 , GD3 , 9-O-acetyl-GD3 , GM2 , GD2 , and GT3 , increased .
	manualset3
202222	17	417500	7	NULL	NULL	0	NULL	ganglio-series structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When NTERA-2 cells were induced to differentiate by culturing in the presence of 10 ( -5 ) M retinoic acid , a remarkable shift of cellular glycolipids from globo-series to lacto - and ganglio-series was observed : Globo-series structures declined , particularly during the period 7-20 days after first exposure to retinoic acid , while lacto-series structures , including fucosyl alpha 1 -- 3 type 2 chain ( Lex ) and sialosyl type 2 chain , and ganglio-series structures , including GM3 , GD3 , 9-O-acetyl-GD3 , GM2 , GD2 , and GT3 , increased .
	manualset3
202223	18	417500	7	NULL	NULL	0	NULL	GM3	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When NTERA-2 cells were induced to differentiate by culturing in the presence of 10 ( -5 ) M retinoic acid , a remarkable shift of cellular glycolipids from globo-series to lacto - and ganglio-series was observed : Globo-series structures declined , particularly during the period 7-20 days after first exposure to retinoic acid , while lacto-series structures , including fucosyl alpha 1 -- 3 type 2 chain ( Lex ) and sialosyl type 2 chain , and ganglio-series structures , including GM3 , GD3 , 9-O-acetyl-GD3 , GM2 , GD2 , and GT3 , increased .
	manualset3
202224	19	417500	7	NULL	NULL	0	NULL	GD3	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When NTERA-2 cells were induced to differentiate by culturing in the presence of 10 ( -5 ) M retinoic acid , a remarkable shift of cellular glycolipids from globo-series to lacto - and ganglio-series was observed : Globo-series structures declined , particularly during the period 7-20 days after first exposure to retinoic acid , while lacto-series structures , including fucosyl alpha 1 -- 3 type 2 chain ( Lex ) and sialosyl type 2 chain , and ganglio-series structures , including GM3 , GD3 , 9-O-acetyl-GD3 , GM2 , GD2 , and GT3 , increased .
	manualset3
202225	20	417500	7	NULL	NULL	0	NULL	9-O-acetyl-GD3	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When NTERA-2 cells were induced to differentiate by culturing in the presence of 10 ( -5 ) M retinoic acid , a remarkable shift of cellular glycolipids from globo-series to lacto - and ganglio-series was observed : Globo-series structures declined , particularly during the period 7-20 days after first exposure to retinoic acid , while lacto-series structures , including fucosyl alpha 1 -- 3 type 2 chain ( Lex ) and sialosyl type 2 chain , and ganglio-series structures , including GM3 , GD3 , 9-O-acetyl-GD3 , GM2 , GD2 , and GT3 , increased .
	manualset3
202226	21	417500	7	NULL	NULL	0	NULL	GM2	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When NTERA-2 cells were induced to differentiate by culturing in the presence of 10 ( -5 ) M retinoic acid , a remarkable shift of cellular glycolipids from globo-series to lacto - and ganglio-series was observed : Globo-series structures declined , particularly during the period 7-20 days after first exposure to retinoic acid , while lacto-series structures , including fucosyl alpha 1 -- 3 type 2 chain ( Lex ) and sialosyl type 2 chain , and ganglio-series structures , including GM3 , GD3 , 9-O-acetyl-GD3 , GM2 , GD2 , and GT3 , increased .
	manualset3
202227	22	417500	7	NULL	NULL	0	NULL	GD2	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When NTERA-2 cells were induced to differentiate by culturing in the presence of 10 ( -5 ) M retinoic acid , a remarkable shift of cellular glycolipids from globo-series to lacto - and ganglio-series was observed : Globo-series structures declined , particularly during the period 7-20 days after first exposure to retinoic acid , while lacto-series structures , including fucosyl alpha 1 -- 3 type 2 chain ( Lex ) and sialosyl type 2 chain , and ganglio-series structures , including GM3 , GD3 , 9-O-acetyl-GD3 , GM2 , GD2 , and GT3 , increased .
	manualset3
202228	23	417500	7	NULL	NULL	0	NULL	GT3	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When NTERA-2 cells were induced to differentiate by culturing in the presence of 10 ( -5 ) M retinoic acid , a remarkable shift of cellular glycolipids from globo-series to lacto - and ganglio-series was observed : Globo-series structures declined , particularly during the period 7-20 days after first exposure to retinoic acid , while lacto-series structures , including fucosyl alpha 1 -- 3 type 2 chain ( Lex ) and sialosyl type 2 chain , and ganglio-series structures , including GM3 , GD3 , 9-O-acetyl-GD3 , GM2 , GD2 , and GT3 , increased .
	manualset3
202229	24	417500	7	NULL	NULL	0	NULL	 lacto -series	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When NTERA-2 cells were induced to differentiate by culturing in the presence of 10 ( -5 ) M retinoic acid , a remarkable shift of cellular glycolipids from globo-series to lacto - and ganglio-series was observed : Globo-series structures declined , particularly during the period 7-20 days after first exposure to retinoic acid , while lacto-series structures , including fucosyl alpha 1 -- 3 type 2 chain ( Lex ) and sialosyl type 2 chain , and ganglio-series structures , including GM3 , GD3 , 9-O-acetyl-GD3 , GM2 , GD2 , and GT3 , increased .
	manualset3
202319	1	417501	7	NULL	NULL	0	NULL	PCA	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	When PCA was applied , different components were obtained for tumorous and non-tumorous tissues .
	manualset3
202320	2	417501	7	NULL	NULL	0	NULL	 components	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When PCA was applied , different components were obtained for tumorous and non-tumorous tissues .
	manualset3
202321	3	417501	7	NULL	NULL	0	NULL	tumorous tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	When PCA was applied , different components were obtained for tumorous and non-tumorous tissues .
	manualset3
202322	4	417501	7	NULL	NULL	0	NULL	non-tumorous tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	When PCA was applied , different components were obtained for tumorous and non-tumorous tissues .
	manualset3
202323	1	417502	7	NULL	NULL	0	NULL	Pkn2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When Pkn2 is inducibly expressed in E. coli , cells are unable to form colonies on agar plates .
	manualset3
202324	2	417502	7	NULL	NULL	0	NULL	E. coli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When Pkn2 is inducibly expressed in E. coli , cells are unable to form colonies on agar plates .
	manualset3
202325	3	417502	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	When Pkn2 is inducibly expressed in E. coli , cells are unable to form colonies on agar plates .
	manualset3
202326	4	417502	7	NULL	NULL	NULL	NULL	colonies	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When Pkn2 is inducibly expressed in E. coli , cells are unable to form colonies on agar plates .
	manualset3
202327	5	417502	7	NULL	NULL	NULL	NULL	agar plates	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When Pkn2 is inducibly expressed in E. coli , cells are unable to form colonies on agar plates .
	manualset3
202328	1	417503	7	NULL	NULL	0	NULL	PomA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When PomA with an introduced Cys residue ( Cys-PomA ) in the C-terminal periplasmic loop ( loop ( 3-4 ) ) was examined without exposure to a reducing reagent , a 43-kDa band was observed , whereas only a 25-kDa band , which corresponds to monomeric PomA , was observed under reducing conditions .
	manualset3
202329	2	417503	7	NULL	NULL	0	NULL	Cys residue	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	When PomA with an introduced Cys residue ( Cys-PomA ) in the C-terminal periplasmic loop ( loop ( 3-4 ) ) was examined without exposure to a reducing reagent , a 43-kDa band was observed , whereas only a 25-kDa band , which corresponds to monomeric PomA , was observed under reducing conditions .
	manualset3
202330	3	417503	7	NULL	NULL	0	NULL	Cys-PomA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When PomA with an introduced Cys residue ( Cys-PomA ) in the C-terminal periplasmic loop ( loop ( 3-4 ) ) was examined without exposure to a reducing reagent , a 43-kDa band was observed , whereas only a 25-kDa band , which corresponds to monomeric PomA , was observed under reducing conditions .
	manualset3
202331	4	417503	7	NULL	NULL	0	NULL	C-terminal periplasmic loop 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	When PomA with an introduced Cys residue ( Cys-PomA ) in the C-terminal periplasmic loop ( loop ( 3-4 ) ) was examined without exposure to a reducing reagent , a 43-kDa band was observed , whereas only a 25-kDa band , which corresponds to monomeric PomA , was observed under reducing conditions .
	manualset3
202332	5	417503	7	NULL	NULL	0	NULL	loop ( 3-4 )	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	When PomA with an introduced Cys residue ( Cys-PomA ) in the C-terminal periplasmic loop ( loop ( 3-4 ) ) was examined without exposure to a reducing reagent , a 43-kDa band was observed , whereas only a 25-kDa band , which corresponds to monomeric PomA , was observed under reducing conditions .
	manualset3
202333	6	417503	7	NULL	NULL	0	NULL	 reducing reagent 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When PomA with an introduced Cys residue ( Cys-PomA ) in the C-terminal periplasmic loop ( loop ( 3-4 ) ) was examined without exposure to a reducing reagent , a 43-kDa band was observed , whereas only a 25-kDa band , which corresponds to monomeric PomA , was observed under reducing conditions .
	manualset3
202334	7	417503	7	NULL	NULL	0	NULL	43-kDa band	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When PomA with an introduced Cys residue ( Cys-PomA ) in the C-terminal periplasmic loop ( loop ( 3-4 ) ) was examined without exposure to a reducing reagent , a 43-kDa band was observed , whereas only a 25-kDa band , which corresponds to monomeric PomA , was observed under reducing conditions .
	manualset3
202335	8	417503	7	NULL	NULL	0	NULL	25-kDa band	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When PomA with an introduced Cys residue ( Cys-PomA ) in the C-terminal periplasmic loop ( loop ( 3-4 ) ) was examined without exposure to a reducing reagent , a 43-kDa band was observed , whereas only a 25-kDa band , which corresponds to monomeric PomA , was observed under reducing conditions .
	manualset3
202336	9	417503	7	NULL	NULL	0	NULL	monomeric PomA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When PomA with an introduced Cys residue ( Cys-PomA ) in the C-terminal periplasmic loop ( loop ( 3-4 ) ) was examined without exposure to a reducing reagent , a 43-kDa band was observed , whereas only a 25-kDa band , which corresponds to monomeric PomA , was observed under reducing conditions .
	manualset3
202337	10	417503	7	NULL	NULL	0	NULL	reducing conditions 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	When PomA with an introduced Cys residue ( Cys-PomA ) in the C-terminal periplasmic loop ( loop ( 3-4 ) ) was examined without exposure to a reducing reagent , a 43-kDa band was observed , whereas only a 25-kDa band , which corresponds to monomeric PomA , was observed under reducing conditions .
	manualset3
202338	1	417504	7	NULL	NULL	0	NULL	Se supplementation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When Se supplementation stops , the liver , kidney , and egg white and yolk residues decline quickly to control values within 1-2 wk .
	manualset3
202339	2	417504	7	NULL	NULL	0	NULL	 liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When Se supplementation stops , the liver , kidney , and egg white and yolk residues decline quickly to control values within 1-2 wk .
	manualset3
202340	3	417504	7	NULL	NULL	0	NULL	kidney	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When Se supplementation stops , the liver , kidney , and egg white and yolk residues decline quickly to control values within 1-2 wk .
	manualset3
202341	4	417504	7	NULL	NULL	0	NULL	egg white	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When Se supplementation stops , the liver , kidney , and egg white and yolk residues decline quickly to control values within 1-2 wk .
	manualset3
202342	5	417504	7	NULL	NULL	0	NULL	yolk residues	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When Se supplementation stops , the liver , kidney , and egg white and yolk residues decline quickly to control values within 1-2 wk .
	manualset3
202343	6	417504	7	NULL	NULL	0	NULL	values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When Se supplementation stops , the liver , kidney , and egg white and yolk residues decline quickly to control values within 1-2 wk .
	manualset3
202344	7	417504	7	NULL	NULL	0	NULL	1-2 wk	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	When Se supplementation stops , the liver , kidney , and egg white and yolk residues decline quickly to control values within 1-2 wk .
	manualset3
202345	1	417505	7	NULL	NULL	0	NULL	UWL	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When UWL was high , Jd of fatty acids was greater in old than in young animals ; Jd was greatly increased when UWL was low , and Jd was not higher in the suckling and mature rather than the old animals .
	manualset3
202346	2	417505	7	NULL	NULL	0	NULL	Jd	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When UWL was high , Jd of fatty acids was greater in old than in young animals ; Jd was greatly increased when UWL was low , and Jd was not higher in the suckling and mature rather than the old animals .
	manualset3
202347	3	417505	7	NULL	NULL	0	NULL	 fatty acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When UWL was high , Jd of fatty acids was greater in old than in young animals ; Jd was greatly increased when UWL was low , and Jd was not higher in the suckling and mature rather than the old animals .
	manualset3
202348	4	417505	7	NULL	NULL	0	NULL	old	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	When UWL was high , Jd of fatty acids was greater in old than in young animals ; Jd was greatly increased when UWL was low , and Jd was not higher in the suckling and mature rather than the old animals .
	manualset3
202349	5	417505	7	NULL	NULL	0	NULL	 young animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When UWL was high , Jd of fatty acids was greater in old than in young animals ; Jd was greatly increased when UWL was low , and Jd was not higher in the suckling and mature rather than the old animals .
	manualset3
202350	6	417505	7	NULL	NULL	0	NULL	Jd	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When UWL was high , Jd of fatty acids was greater in old than in young animals ; Jd was greatly increased when UWL was low , and Jd was not higher in the suckling and mature rather than the old animals .
	manualset3
202351	7	417505	7	NULL	NULL	0	NULL	UWL	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When UWL was high , Jd of fatty acids was greater in old than in young animals ; Jd was greatly increased when UWL was low , and Jd was not higher in the suckling and mature rather than the old animals .
	manualset3
202352	8	417505	7	NULL	NULL	0	NULL	Jd	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When UWL was high , Jd of fatty acids was greater in old than in young animals ; Jd was greatly increased when UWL was low , and Jd was not higher in the suckling and mature rather than the old animals .
	manualset3
202353	9	417505	7	NULL	NULL	0	NULL	suckling	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When UWL was high , Jd of fatty acids was greater in old than in young animals ; Jd was greatly increased when UWL was low , and Jd was not higher in the suckling and mature rather than the old animals .
	manualset3
202354	10	417505	7	NULL	NULL	0	NULL	mature	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When UWL was high , Jd of fatty acids was greater in old than in young animals ; Jd was greatly increased when UWL was low , and Jd was not higher in the suckling and mature rather than the old animals .
	manualset3
202355	11	417505	7	NULL	NULL	0	NULL	old animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When UWL was high , Jd of fatty acids was greater in old than in young animals ; Jd was greatly increased when UWL was low , and Jd was not higher in the suckling and mature rather than the old animals .
	manualset3
202356	1	417506	7	NULL	NULL	0	NULL	cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	When a cell was dialyzed with pipette solution containing 100 micro M cGMP , I ( Ks ) started to gradually increase and reached a maximum increase of a factor of 2.37 + / - 0.39 ( n = 4 ) about 10-15 min after rupture of patch membrane .
	manualset3
202357	2	417506	7	NULL	NULL	0	NULL	 pipette solution 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When a cell was dialyzed with pipette solution containing 100 micro M cGMP , I ( Ks ) started to gradually increase and reached a maximum increase of a factor of 2.37 + / - 0.39 ( n = 4 ) about 10-15 min after rupture of patch membrane .
	manualset3
202358	3	417506	7	NULL	NULL	NULL	NULL	100 micro M	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When a cell was dialyzed with pipette solution containing 100 micro M cGMP , I ( Ks ) started to gradually increase and reached a maximum increase of a factor of 2.37 + / - 0.39 ( n = 4 ) about 10-15 min after rupture of patch membrane .
	manualset3
202359	4	417506	7	NULL	NULL	NULL	NULL	cGMP	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When a cell was dialyzed with pipette solution containing 100 micro M cGMP , I ( Ks ) started to gradually increase and reached a maximum increase of a factor of 2.37 + / - 0.39 ( n = 4 ) about 10-15 min after rupture of patch membrane .
	manualset3
202360	5	417506	7	NULL	NULL	0	NULL	 I ( Ks )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When a cell was dialyzed with pipette solution containing 100 micro M cGMP , I ( Ks ) started to gradually increase and reached a maximum increase of a factor of 2.37 + / - 0.39 ( n = 4 ) about 10-15 min after rupture of patch membrane .
	manualset3
202361	6	417506	7	NULL	NULL	0	NULL	maximum increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When a cell was dialyzed with pipette solution containing 100 micro M cGMP , I ( Ks ) started to gradually increase and reached a maximum increase of a factor of 2.37 + / - 0.39 ( n = 4 ) about 10-15 min after rupture of patch membrane .
	manualset3
202362	7	417506	7	NULL	NULL	0	NULL	 factor	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When a cell was dialyzed with pipette solution containing 100 micro M cGMP , I ( Ks ) started to gradually increase and reached a maximum increase of a factor of 2.37 + / - 0.39 ( n = 4 ) about 10-15 min after rupture of patch membrane .
	manualset3
202363	8	417506	7	NULL	NULL	0	NULL	2.37 + / - 0.39	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	When a cell was dialyzed with pipette solution containing 100 micro M cGMP , I ( Ks ) started to gradually increase and reached a maximum increase of a factor of 2.37 + / - 0.39 ( n = 4 ) about 10-15 min after rupture of patch membrane .
	manualset3
202364	9	417506	7	NULL	NULL	0	NULL	 n = 4	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When a cell was dialyzed with pipette solution containing 100 micro M cGMP , I ( Ks ) started to gradually increase and reached a maximum increase of a factor of 2.37 + / - 0.39 ( n = 4 ) about 10-15 min after rupture of patch membrane .
	manualset3
202365	10	417506	7	NULL	NULL	0	NULL	10-15 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	When a cell was dialyzed with pipette solution containing 100 micro M cGMP , I ( Ks ) started to gradually increase and reached a maximum increase of a factor of 2.37 + / - 0.39 ( n = 4 ) about 10-15 min after rupture of patch membrane .
	manualset3
202366	11	417506	7	NULL	NULL	0	NULL	rupture	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When a cell was dialyzed with pipette solution containing 100 micro M cGMP , I ( Ks ) started to gradually increase and reached a maximum increase of a factor of 2.37 + / - 0.39 ( n = 4 ) about 10-15 min after rupture of patch membrane .
	manualset3
202367	12	417506	7	NULL	NULL	0	NULL	patch membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	When a cell was dialyzed with pipette solution containing 100 micro M cGMP , I ( Ks ) started to gradually increase and reached a maximum increase of a factor of 2.37 + / - 0.39 ( n = 4 ) about 10-15 min after rupture of patch membrane .
	manualset3
202496	1	417507	7	NULL	NULL	0	NULL	drug product	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	When a drug product is dosed via drinking water in a farm setting , a number of variables , including pH , chlorine content , hardness of the water used for dilution , and container material , may affect its stability , leading to a decrease in drug potency .
	manualset3
202499	2	417507	7	NULL	NULL	0	NULL	drinking water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When a drug product is dosed via drinking water in a farm setting , a number of variables , including pH , chlorine content , hardness of the water used for dilution , and container material , may affect its stability , leading to a decrease in drug potency .
	manualset3
202501	3	417507	7	NULL	NULL	0	NULL	 farm setting	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	When a drug product is dosed via drinking water in a farm setting , a number of variables , including pH , chlorine content , hardness of the water used for dilution , and container material , may affect its stability , leading to a decrease in drug potency .
	manualset3
202502	4	417507	7	NULL	NULL	0	NULL	 number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When a drug product is dosed via drinking water in a farm setting , a number of variables , including pH , chlorine content , hardness of the water used for dilution , and container material , may affect its stability , leading to a decrease in drug potency .
	manualset3
202504	5	417507	7	NULL	NULL	0	NULL	variables	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When a drug product is dosed via drinking water in a farm setting , a number of variables , including pH , chlorine content , hardness of the water used for dilution , and container material , may affect its stability , leading to a decrease in drug potency .
	manualset3
202507	6	417507	7	NULL	NULL	0	NULL	pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When a drug product is dosed via drinking water in a farm setting , a number of variables , including pH , chlorine content , hardness of the water used for dilution , and container material , may affect its stability , leading to a decrease in drug potency .
	manualset3
202508	7	417507	7	NULL	NULL	0	NULL	chlorine content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When a drug product is dosed via drinking water in a farm setting , a number of variables , including pH , chlorine content , hardness of the water used for dilution , and container material , may affect its stability , leading to a decrease in drug potency .
	manualset3
202510	8	417507	7	NULL	NULL	0	NULL	hardness	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When a drug product is dosed via drinking water in a farm setting , a number of variables , including pH , chlorine content , hardness of the water used for dilution , and container material , may affect its stability , leading to a decrease in drug potency .
	manualset3
202511	9	417507	7	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When a drug product is dosed via drinking water in a farm setting , a number of variables , including pH , chlorine content , hardness of the water used for dilution , and container material , may affect its stability , leading to a decrease in drug potency .
	manualset3
202513	10	417507	7	NULL	NULL	0	NULL	dilution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When a drug product is dosed via drinking water in a farm setting , a number of variables , including pH , chlorine content , hardness of the water used for dilution , and container material , may affect its stability , leading to a decrease in drug potency .
	manualset3
202514	11	417507	7	NULL	NULL	0	NULL	container material 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When a drug product is dosed via drinking water in a farm setting , a number of variables , including pH , chlorine content , hardness of the water used for dilution , and container material , may affect its stability , leading to a decrease in drug potency .
	manualset3
202518	12	417507	7	NULL	NULL	0	NULL	stability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When a drug product is dosed via drinking water in a farm setting , a number of variables , including pH , chlorine content , hardness of the water used for dilution , and container material , may affect its stability , leading to a decrease in drug potency .
	manualset3
202519	13	417507	7	NULL	NULL	0	NULL	drug potency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When a drug product is dosed via drinking water in a farm setting , a number of variables , including pH , chlorine content , hardness of the water used for dilution , and container material , may affect its stability , leading to a decrease in drug potency .
	manualset3
202520	1	417508	7	NULL	NULL	NULL	NULL	single filament	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When a single filament is allowed to grow in a bath of constant concentration of free ADP-actin monomers , its growth rate increases linearly with the free monomer concentration in quantitative agreement with in vitro experiments .
	manualset3
202521	2	417508	7	NULL	NULL	0	NULL	bath	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	When a single filament is allowed to grow in a bath of constant concentration of free ADP-actin monomers , its growth rate increases linearly with the free monomer concentration in quantitative agreement with in vitro experiments .
	manualset3
202522	3	417508	7	NULL	NULL	0	NULL	constant concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When a single filament is allowed to grow in a bath of constant concentration of free ADP-actin monomers , its growth rate increases linearly with the free monomer concentration in quantitative agreement with in vitro experiments .
	manualset3
202523	4	417508	7	NULL	NULL	0	NULL	free ADP-actin monomers	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When a single filament is allowed to grow in a bath of constant concentration of free ADP-actin monomers , its growth rate increases linearly with the free monomer concentration in quantitative agreement with in vitro experiments .
	manualset3
202524	5	417508	7	NULL	NULL	0	NULL	growth rate 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When a single filament is allowed to grow in a bath of constant concentration of free ADP-actin monomers , its growth rate increases linearly with the free monomer concentration in quantitative agreement with in vitro experiments .
	manualset3
202525	6	417508	7	NULL	NULL	0	NULL	 free monomer concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When a single filament is allowed to grow in a bath of constant concentration of free ADP-actin monomers , its growth rate increases linearly with the free monomer concentration in quantitative agreement with in vitro experiments .
	manualset3
202526	7	417508	7	NULL	NULL	0	NULL	quantitative agreement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When a single filament is allowed to grow in a bath of constant concentration of free ADP-actin monomers , its growth rate increases linearly with the free monomer concentration in quantitative agreement with in vitro experiments .
	manualset3
202527	8	417508	7	NULL	NULL	0	NULL	in vitro experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	When a single filament is allowed to grow in a bath of constant concentration of free ADP-actin monomers , its growth rate increases linearly with the free monomer concentration in quantitative agreement with in vitro experiments .
	manualset3
202528	1	417509	7	NULL	NULL	0	NULL	two-step reverse transcription PCR amplification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	When a two-step reverse transcription PCR amplification is employed , the device can detect ribonucleic acid ( RNA ) analogs of all four viral targets with detection limits in the range of 25-100 copies/reactor .
	manualset3
202529	2	417509	7	NULL	NULL	0	NULL	device	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	When a two-step reverse transcription PCR amplification is employed , the device can detect ribonucleic acid ( RNA ) analogs of all four viral targets with detection limits in the range of 25-100 copies/reactor .
	manualset3
202530	3	417509	7	NULL	NULL	0	NULL	ribonucleic acid ( RNA ) analogs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	When a two-step reverse transcription PCR amplification is employed , the device can detect ribonucleic acid ( RNA ) analogs of all four viral targets with detection limits in the range of 25-100 copies/reactor .
	manualset3
202531	4	417509	7	NULL	NULL	0	NULL	 four viral targets	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When a two-step reverse transcription PCR amplification is employed , the device can detect ribonucleic acid ( RNA ) analogs of all four viral targets with detection limits in the range of 25-100 copies/reactor .
	manualset3
202532	5	417509	7	NULL	NULL	0	NULL	detection limits	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When a two-step reverse transcription PCR amplification is employed , the device can detect ribonucleic acid ( RNA ) analogs of all four viral targets with detection limits in the range of 25-100 copies/reactor .
	manualset3
202533	6	417509	7	NULL	NULL	0	NULL	range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When a two-step reverse transcription PCR amplification is employed , the device can detect ribonucleic acid ( RNA ) analogs of all four viral targets with detection limits in the range of 25-100 copies/reactor .
	manualset3
202534	7	417509	7	NULL	NULL	0	NULL	25-100 copies/reactor	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	When a two-step reverse transcription PCR amplification is employed , the device can detect ribonucleic acid ( RNA ) analogs of all four viral targets with detection limits in the range of 25-100 copies/reactor .
	manualset3
202535	1	417510	7	NULL	NULL	0	NULL	age	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	When adjusted for age , which was the most important factor affecting outcome , the presence of a ras mutation emerged as a significant predictor for improved survival ( P = .03 ) and along with lower bone marrow blast counts ( P = .02 ) and better cytogenetic category ( P = .01 ) .
	manualset3
202536	2	417510	7	NULL	NULL	NULL	NULL	factor	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When adjusted for age , which was the most important factor affecting outcome , the presence of a ras mutation emerged as a significant predictor for improved survival ( P = .03 ) and along with lower bone marrow blast counts ( P = .02 ) and better cytogenetic category ( P = .01 ) .
	manualset3
202537	3	417510	7	NULL	NULL	0	NULL	outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When adjusted for age , which was the most important factor affecting outcome , the presence of a ras mutation emerged as a significant predictor for improved survival ( P = .03 ) and along with lower bone marrow blast counts ( P = .02 ) and better cytogenetic category ( P = .01 ) .
	manualset3
202538	4	417510	7	NULL	NULL	NULL	NULL	ras mutation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When adjusted for age , which was the most important factor affecting outcome , the presence of a ras mutation emerged as a significant predictor for improved survival ( P = .03 ) and along with lower bone marrow blast counts ( P = .02 ) and better cytogenetic category ( P = .01 ) .
	manualset3
202539	5	417510	7	NULL	NULL	NULL	NULL	predictor	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When adjusted for age , which was the most important factor affecting outcome , the presence of a ras mutation emerged as a significant predictor for improved survival ( P = .03 ) and along with lower bone marrow blast counts ( P = .02 ) and better cytogenetic category ( P = .01 ) .
	manualset3
202540	6	417510	7	NULL	NULL	0	NULL	improved survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When adjusted for age , which was the most important factor affecting outcome , the presence of a ras mutation emerged as a significant predictor for improved survival ( P = .03 ) and along with lower bone marrow blast counts ( P = .02 ) and better cytogenetic category ( P = .01 ) .
	manualset3
202541	7	417510	7	NULL	NULL	0	NULL	P = .03	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	When adjusted for age , which was the most important factor affecting outcome , the presence of a ras mutation emerged as a significant predictor for improved survival ( P = .03 ) and along with lower bone marrow blast counts ( P = .02 ) and better cytogenetic category ( P = .01 ) .
	manualset3
202542	8	417510	7	NULL	NULL	0	NULL	lower bone marrow blast counts 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When adjusted for age , which was the most important factor affecting outcome , the presence of a ras mutation emerged as a significant predictor for improved survival ( P = .03 ) and along with lower bone marrow blast counts ( P = .02 ) and better cytogenetic category ( P = .01 ) .
	manualset3
202543	9	417510	7	NULL	NULL	0	NULL	P = .02	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	When adjusted for age , which was the most important factor affecting outcome , the presence of a ras mutation emerged as a significant predictor for improved survival ( P = .03 ) and along with lower bone marrow blast counts ( P = .02 ) and better cytogenetic category ( P = .01 ) .
	manualset3
202544	10	417510	7	NULL	NULL	0	NULL	cytogenetic category	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When adjusted for age , which was the most important factor affecting outcome , the presence of a ras mutation emerged as a significant predictor for improved survival ( P = .03 ) and along with lower bone marrow blast counts ( P = .02 ) and better cytogenetic category ( P = .01 ) .
	manualset3
202545	11	417510	7	NULL	NULL	0	NULL	P = .01 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	When adjusted for age , which was the most important factor affecting outcome , the presence of a ras mutation emerged as a significant predictor for improved survival ( P = .03 ) and along with lower bone marrow blast counts ( P = .02 ) and better cytogenetic category ( P = .01 ) .
	manualset3
202546	1	417511	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	When all data of eta versus IMT of NTA and HTA were pooled in a linear regression analysis , a correlation coefficient of r = .71 ( P & lt ; .05 ) was obtained .
	manualset3
202547	2	417511	7	NULL	NULL	0	NULL	eta 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When all data of eta versus IMT of NTA and HTA were pooled in a linear regression analysis , a correlation coefficient of r = .71 ( P & lt ; .05 ) was obtained .
	manualset3
202548	3	417511	7	NULL	NULL	0	NULL	 IMT 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When all data of eta versus IMT of NTA and HTA were pooled in a linear regression analysis , a correlation coefficient of r = .71 ( P & lt ; .05 ) was obtained .
	manualset3
202549	4	417511	7	NULL	NULL	0	NULL	NTA	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When all data of eta versus IMT of NTA and HTA were pooled in a linear regression analysis , a correlation coefficient of r = .71 ( P & lt ; .05 ) was obtained .
	manualset3
202550	5	417511	7	NULL	NULL	0	NULL	HTA	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When all data of eta versus IMT of NTA and HTA were pooled in a linear regression analysis , a correlation coefficient of r = .71 ( P & lt ; .05 ) was obtained .
	manualset3
202551	6	417511	7	NULL	NULL	0	NULL	linear regression analysis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	When all data of eta versus IMT of NTA and HTA were pooled in a linear regression analysis , a correlation coefficient of r = .71 ( P & lt ; .05 ) was obtained .
	manualset3
202552	7	417511	7	NULL	NULL	0	NULL	correlation coefficient	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When all data of eta versus IMT of NTA and HTA were pooled in a linear regression analysis , a correlation coefficient of r = .71 ( P & lt ; .05 ) was obtained .
	manualset3
202553	8	417511	7	NULL	NULL	0	NULL	 r = .71	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	When all data of eta versus IMT of NTA and HTA were pooled in a linear regression analysis , a correlation coefficient of r = .71 ( P & lt ; .05 ) was obtained .
	manualset3
202554	9	417511	7	NULL	NULL	0	NULL	P & lt ; .05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	When all data of eta versus IMT of NTA and HTA were pooled in a linear regression analysis , a correlation coefficient of r = .71 ( P & lt ; .05 ) was obtained .
	manualset3
202555	1	417512	7	NULL	NULL	0	NULL	in-line Fresnel hologram	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	When an in-line Fresnel hologram of an object such as a projectile in flight is made , the reconstruction comprises an image of the outside edge of the object superimposed upon a Fresnel diffraction pattern of the edge and an unmodulated portion of the reconstruction beam .
	manualset3
202556	2	417512	7	NULL	NULL	0	NULL	object	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When an in-line Fresnel hologram of an object such as a projectile in flight is made , the reconstruction comprises an image of the outside edge of the object superimposed upon a Fresnel diffraction pattern of the edge and an unmodulated portion of the reconstruction beam .
	manualset3
202557	3	417512	7	NULL	NULL	0	NULL	 projectile	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When an in-line Fresnel hologram of an object such as a projectile in flight is made , the reconstruction comprises an image of the outside edge of the object superimposed upon a Fresnel diffraction pattern of the edge and an unmodulated portion of the reconstruction beam .
	manualset3
202558	4	417512	7	NULL	NULL	NULL	NULL	flight	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When an in-line Fresnel hologram of an object such as a projectile in flight is made , the reconstruction comprises an image of the outside edge of the object superimposed upon a Fresnel diffraction pattern of the edge and an unmodulated portion of the reconstruction beam .
	manualset3
202559	5	417512	7	NULL	NULL	0	NULL	reconstruction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When an in-line Fresnel hologram of an object such as a projectile in flight is made , the reconstruction comprises an image of the outside edge of the object superimposed upon a Fresnel diffraction pattern of the edge and an unmodulated portion of the reconstruction beam .
	manualset3
202560	6	417512	7	NULL	NULL	0	NULL	image	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When an in-line Fresnel hologram of an object such as a projectile in flight is made , the reconstruction comprises an image of the outside edge of the object superimposed upon a Fresnel diffraction pattern of the edge and an unmodulated portion of the reconstruction beam .
	manualset3
202561	7	417512	7	NULL	NULL	0	NULL	outside edge	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When an in-line Fresnel hologram of an object such as a projectile in flight is made , the reconstruction comprises an image of the outside edge of the object superimposed upon a Fresnel diffraction pattern of the edge and an unmodulated portion of the reconstruction beam .
	manualset3
202562	8	417512	7	NULL	NULL	0	NULL	object	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When an in-line Fresnel hologram of an object such as a projectile in flight is made , the reconstruction comprises an image of the outside edge of the object superimposed upon a Fresnel diffraction pattern of the edge and an unmodulated portion of the reconstruction beam .
	manualset3
202563	9	417512	7	NULL	NULL	0	NULL	Fresnel diffraction pattern	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	When an in-line Fresnel hologram of an object such as a projectile in flight is made , the reconstruction comprises an image of the outside edge of the object superimposed upon a Fresnel diffraction pattern of the edge and an unmodulated portion of the reconstruction beam .
	manualset3
202564	10	417512	7	NULL	NULL	0	NULL	edge 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When an in-line Fresnel hologram of an object such as a projectile in flight is made , the reconstruction comprises an image of the outside edge of the object superimposed upon a Fresnel diffraction pattern of the edge and an unmodulated portion of the reconstruction beam .
	manualset3
202565	11	417512	7	NULL	NULL	0	NULL	unmodulated portion	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	When an in-line Fresnel hologram of an object such as a projectile in flight is made , the reconstruction comprises an image of the outside edge of the object superimposed upon a Fresnel diffraction pattern of the edge and an unmodulated portion of the reconstruction beam .
	manualset3
202566	12	417512	7	NULL	NULL	0	NULL	 reconstruction beam	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	When an in-line Fresnel hologram of an object such as a projectile in flight is made , the reconstruction comprises an image of the outside edge of the object superimposed upon a Fresnel diffraction pattern of the edge and an unmodulated portion of the reconstruction beam .
	manualset3
202567	1	417513	7	NULL	NULL	0	NULL	infusion fluid drop	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	When an infusion fluid drop is forming , its length and diameter , and therefore the drip chamber capacitance , are increasing , causing change in the output signal .
	manualset3
202568	2	417513	7	NULL	NULL	0	NULL	length	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When an infusion fluid drop is forming , its length and diameter , and therefore the drip chamber capacitance , are increasing , causing change in the output signal .
	manualset3
202569	3	417513	7	NULL	NULL	0	NULL	diameter	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When an infusion fluid drop is forming , its length and diameter , and therefore the drip chamber capacitance , are increasing , causing change in the output signal .
	manualset3
202570	4	417513	7	NULL	NULL	0	NULL	drip chamber capacitance	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	When an infusion fluid drop is forming , its length and diameter , and therefore the drip chamber capacitance , are increasing , causing change in the output signal .
	manualset3
202571	5	417513	7	NULL	NULL	0	NULL	 change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When an infusion fluid drop is forming , its length and diameter , and therefore the drip chamber capacitance , are increasing , causing change in the output signal .
	manualset3
202572	6	417513	7	NULL	NULL	0	NULL	output signal	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When an infusion fluid drop is forming , its length and diameter , and therefore the drip chamber capacitance , are increasing , causing change in the output signal .
	manualset3
202573	1	417514	7	NULL	NULL	0	NULL	 embryos	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When analyzed in embryos cultured without serum , the dynamics of the different mitochondrial types appeared to be similar , a fact that may provide evidence that the developmental changes control the mitochondrial dynamics , and that swollen mitochondria may not be completely inactive .
	manualset3
202574	2	417514	7	NULL	NULL	NULL	NULL	serum	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When analyzed in embryos cultured without serum , the dynamics of the different mitochondrial types appeared to be similar , a fact that may provide evidence that the developmental changes control the mitochondrial dynamics , and that swollen mitochondria may not be completely inactive .
	manualset3
202575	3	417514	7	NULL	NULL	NULL	NULL	dynamics	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When analyzed in embryos cultured without serum , the dynamics of the different mitochondrial types appeared to be similar , a fact that may provide evidence that the developmental changes control the mitochondrial dynamics , and that swollen mitochondria may not be completely inactive .
	manualset3
202576	4	417514	7	NULL	NULL	0	NULL	different mitochondrial types	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	When analyzed in embryos cultured without serum , the dynamics of the different mitochondrial types appeared to be similar , a fact that may provide evidence that the developmental changes control the mitochondrial dynamics , and that swollen mitochondria may not be completely inactive .
	manualset3
202577	5	417514	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When analyzed in embryos cultured without serum , the dynamics of the different mitochondrial types appeared to be similar , a fact that may provide evidence that the developmental changes control the mitochondrial dynamics , and that swollen mitochondria may not be completely inactive .
	manualset3
202578	6	417514	7	NULL	NULL	0	NULL	developmental changes 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When analyzed in embryos cultured without serum , the dynamics of the different mitochondrial types appeared to be similar , a fact that may provide evidence that the developmental changes control the mitochondrial dynamics , and that swollen mitochondria may not be completely inactive .
	manualset3
202579	7	417514	7	NULL	NULL	0	NULL	mitochondrial dynamics	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When analyzed in embryos cultured without serum , the dynamics of the different mitochondrial types appeared to be similar , a fact that may provide evidence that the developmental changes control the mitochondrial dynamics , and that swollen mitochondria may not be completely inactive .
	manualset3
202580	8	417514	7	NULL	NULL	0	NULL	swollen mitochondria	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	When analyzed in embryos cultured without serum , the dynamics of the different mitochondrial types appeared to be similar , a fact that may provide evidence that the developmental changes control the mitochondrial dynamics , and that swollen mitochondria may not be completely inactive .
	manualset3
204485	9	417514	7	NULL	NULL	0	NULL	fact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When analyzed in embryos cultured without serum , the dynamics of the different mitochondrial types appeared to be similar , a fact that may provide evidence that the developmental changes control the mitochondrial dynamics , and that swollen mitochondria may not be completely inactive .
	manualset3
202581	1	417515	7	NULL	NULL	0	NULL	receptor	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When any receptor in the membrane is aggregated by an external multivalent ligand , the aggregate binds effectively to X , whereas unaggregated receptors do not bind to X. The receptor aggregates , linked to actin ( and myosin ) through X , are then actively collected into a cap by an analog of the actin -- myosin sliding filament mechanism of muscle contraction .
	manualset3
202582	2	417515	7	NULL	NULL	0	NULL	membrane 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	When any receptor in the membrane is aggregated by an external multivalent ligand , the aggregate binds effectively to X , whereas unaggregated receptors do not bind to X. The receptor aggregates , linked to actin ( and myosin ) through X , are then actively collected into a cap by an analog of the actin -- myosin sliding filament mechanism of muscle contraction .
	manualset3
202583	3	417515	7	NULL	NULL	0	NULL	external multivalent ligand	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When any receptor in the membrane is aggregated by an external multivalent ligand , the aggregate binds effectively to X , whereas unaggregated receptors do not bind to X. The receptor aggregates , linked to actin ( and myosin ) through X , are then actively collected into a cap by an analog of the actin -- myosin sliding filament mechanism of muscle contraction .
	manualset3
202584	4	417515	7	NULL	NULL	0	NULL	aggregate	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When any receptor in the membrane is aggregated by an external multivalent ligand , the aggregate binds effectively to X , whereas unaggregated receptors do not bind to X. The receptor aggregates , linked to actin ( and myosin ) through X , are then actively collected into a cap by an analog of the actin -- myosin sliding filament mechanism of muscle contraction .
	manualset3
202585	5	417515	7	NULL	NULL	0	NULL	X	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When any receptor in the membrane is aggregated by an external multivalent ligand , the aggregate binds effectively to X , whereas unaggregated receptors do not bind to X. The receptor aggregates , linked to actin ( and myosin ) through X , are then actively collected into a cap by an analog of the actin -- myosin sliding filament mechanism of muscle contraction .
	manualset3
202586	6	417515	7	NULL	NULL	0	NULL	unaggregated receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When any receptor in the membrane is aggregated by an external multivalent ligand , the aggregate binds effectively to X , whereas unaggregated receptors do not bind to X. The receptor aggregates , linked to actin ( and myosin ) through X , are then actively collected into a cap by an analog of the actin -- myosin sliding filament mechanism of muscle contraction .
	manualset3
202587	7	417515	7	NULL	NULL	0	NULL	X	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When any receptor in the membrane is aggregated by an external multivalent ligand , the aggregate binds effectively to X , whereas unaggregated receptors do not bind to X. The receptor aggregates , linked to actin ( and myosin ) through X , are then actively collected into a cap by an analog of the actin -- myosin sliding filament mechanism of muscle contraction .
	manualset3
202588	8	417515	7	NULL	NULL	0	NULL	receptor aggregates	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When any receptor in the membrane is aggregated by an external multivalent ligand , the aggregate binds effectively to X , whereas unaggregated receptors do not bind to X. The receptor aggregates , linked to actin ( and myosin ) through X , are then actively collected into a cap by an analog of the actin -- myosin sliding filament mechanism of muscle contraction .
	manualset3
202589	9	417515	7	NULL	NULL	0	NULL	actin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When any receptor in the membrane is aggregated by an external multivalent ligand , the aggregate binds effectively to X , whereas unaggregated receptors do not bind to X. The receptor aggregates , linked to actin ( and myosin ) through X , are then actively collected into a cap by an analog of the actin -- myosin sliding filament mechanism of muscle contraction .
	manualset3
202590	10	417515	7	NULL	NULL	0	NULL	myosin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When any receptor in the membrane is aggregated by an external multivalent ligand , the aggregate binds effectively to X , whereas unaggregated receptors do not bind to X. The receptor aggregates , linked to actin ( and myosin ) through X , are then actively collected into a cap by an analog of the actin -- myosin sliding filament mechanism of muscle contraction .
	manualset3
202591	11	417515	7	NULL	NULL	0	NULL	X	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When any receptor in the membrane is aggregated by an external multivalent ligand , the aggregate binds effectively to X , whereas unaggregated receptors do not bind to X. The receptor aggregates , linked to actin ( and myosin ) through X , are then actively collected into a cap by an analog of the actin -- myosin sliding filament mechanism of muscle contraction .
	manualset3
202592	12	417515	7	NULL	NULL	0	NULL	 cap	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When any receptor in the membrane is aggregated by an external multivalent ligand , the aggregate binds effectively to X , whereas unaggregated receptors do not bind to X. The receptor aggregates , linked to actin ( and myosin ) through X , are then actively collected into a cap by an analog of the actin -- myosin sliding filament mechanism of muscle contraction .
	manualset3
202593	13	417515	7	NULL	NULL	0	NULL	analog of the actin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When any receptor in the membrane is aggregated by an external multivalent ligand , the aggregate binds effectively to X , whereas unaggregated receptors do not bind to X. The receptor aggregates , linked to actin ( and myosin ) through X , are then actively collected into a cap by an analog of the actin -- myosin sliding filament mechanism of muscle contraction .
	manualset3
202594	14	417515	7	NULL	NULL	0	NULL	myosin sliding filament mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When any receptor in the membrane is aggregated by an external multivalent ligand , the aggregate binds effectively to X , whereas unaggregated receptors do not bind to X. The receptor aggregates , linked to actin ( and myosin ) through X , are then actively collected into a cap by an analog of the actin -- myosin sliding filament mechanism of muscle contraction .
	manualset3
202595	15	417515	7	NULL	NULL	0	NULL	muscle contraction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When any receptor in the membrane is aggregated by an external multivalent ligand , the aggregate binds effectively to X , whereas unaggregated receptors do not bind to X. The receptor aggregates , linked to actin ( and myosin ) through X , are then actively collected into a cap by an analog of the actin -- myosin sliding filament mechanism of muscle contraction .
	manualset3
202596	1	417516	7	NULL	NULL	0	NULL	proximal pole 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When applied to the proximal pole of the scaphoid , this showed the venous drainage to be via the dorsal ridge into the venae comitantes of the radial artery .
	manualset3
202597	2	417516	7	NULL	NULL	0	NULL	scaphoid	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When applied to the proximal pole of the scaphoid , this showed the venous drainage to be via the dorsal ridge into the venae comitantes of the radial artery .
	manualset3
202598	3	417516	7	NULL	NULL	0	NULL	venous drainage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When applied to the proximal pole of the scaphoid , this showed the venous drainage to be via the dorsal ridge into the venae comitantes of the radial artery .
	manualset3
202599	4	417516	7	NULL	NULL	0	NULL	dorsal ridge 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When applied to the proximal pole of the scaphoid , this showed the venous drainage to be via the dorsal ridge into the venae comitantes of the radial artery .
	manualset3
202600	5	417516	7	NULL	NULL	0	NULL	venae comitantes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When applied to the proximal pole of the scaphoid , this showed the venous drainage to be via the dorsal ridge into the venae comitantes of the radial artery .
	manualset3
202601	6	417516	7	NULL	NULL	0	NULL	radial artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When applied to the proximal pole of the scaphoid , this showed the venous drainage to be via the dorsal ridge into the venae comitantes of the radial artery .
	manualset3
202602	1	417517	7	NULL	NULL	0	NULL	bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When bacteria were infected with either lambda CI857CII2002 or lambda CI857cro27 at low m.o.i. , the usual 65 % -75 % decrease in the percentage of c.c. phage DNA occurred during incubation .
	manualset3
202603	2	417517	7	NULL	NULL	0	NULL	lambda CI857CII2002	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	When bacteria were infected with either lambda CI857CII2002 or lambda CI857cro27 at low m.o.i. , the usual 65 % -75 % decrease in the percentage of c.c. phage DNA occurred during incubation .
	manualset3
202604	3	417517	7	NULL	NULL	0	NULL	lambda CI857cro27	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	When bacteria were infected with either lambda CI857CII2002 or lambda CI857cro27 at low m.o.i. , the usual 65 % -75 % decrease in the percentage of c.c. phage DNA occurred during incubation .
	manualset3
202605	4	417517	7	NULL	NULL	0	NULL	low m.o.i.	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When bacteria were infected with either lambda CI857CII2002 or lambda CI857cro27 at low m.o.i. , the usual 65 % -75 % decrease in the percentage of c.c. phage DNA occurred during incubation .
	manualset3
202606	5	417517	7	NULL	NULL	0	NULL	 65 % -75 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When bacteria were infected with either lambda CI857CII2002 or lambda CI857cro27 at low m.o.i. , the usual 65 % -75 % decrease in the percentage of c.c. phage DNA occurred during incubation .
	manualset3
202607	6	417517	7	NULL	NULL	0	NULL	percentage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When bacteria were infected with either lambda CI857CII2002 or lambda CI857cro27 at low m.o.i. , the usual 65 % -75 % decrease in the percentage of c.c. phage DNA occurred during incubation .
	manualset3
202608	7	417517	7	NULL	NULL	0	NULL	c.c. phage DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	When bacteria were infected with either lambda CI857CII2002 or lambda CI857cro27 at low m.o.i. , the usual 65 % -75 % decrease in the percentage of c.c. phage DNA occurred during incubation .
	manualset3
202609	8	417517	7	NULL	NULL	0	NULL	incubation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	When bacteria were infected with either lambda CI857CII2002 or lambda CI857cro27 at low m.o.i. , the usual 65 % -75 % decrease in the percentage of c.c. phage DNA occurred during incubation .
	manualset3
202610	1	417518	7	NULL	NULL	0	NULL	bacteriuria	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When bacteriuria continues , further examination should be performed for an organic disease of the urinary tract or an overimmunosuppressed state .
	manualset3
202611	2	417518	7	NULL	NULL	NULL	NULL	examination	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When bacteriuria continues , further examination should be performed for an organic disease of the urinary tract or an overimmunosuppressed state .
	manualset3
202612	3	417518	7	NULL	NULL	0	NULL	organic disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	When bacteriuria continues , further examination should be performed for an organic disease of the urinary tract or an overimmunosuppressed state .
	manualset3
202613	4	417518	7	NULL	NULL	0	NULL	urinary tract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When bacteriuria continues , further examination should be performed for an organic disease of the urinary tract or an overimmunosuppressed state .
	manualset3
202614	5	417518	7	NULL	NULL	0	NULL	overimmunosuppressed state	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When bacteriuria continues , further examination should be performed for an organic disease of the urinary tract or an overimmunosuppressed state .
	manualset3
202615	1	417519	7	NULL	NULL	0	NULL	Cortisone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cortisone , ACTH and infections ) .
	manualset3
202616	2	417519	7	NULL	NULL	0	NULL	ACTH	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cortisone , ACTH and infections ) .
	manualset3
202617	3	417519	7	NULL	NULL	0	NULL	infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cortisone , ACTH and infections ) .
	manualset3
202618	1	417520	7	NULL	NULL	0	NULL	beating	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When beating ceased due to verapamil the effect was not reversed by the addition of calcium to the medium .
	manualset3
202619	2	417520	7	NULL	NULL	0	NULL	verapamil	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	When beating ceased due to verapamil the effect was not reversed by the addition of calcium to the medium .
	manualset3
202620	3	417520	7	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When beating ceased due to verapamil the effect was not reversed by the addition of calcium to the medium .
	manualset3
202621	4	417520	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When beating ceased due to verapamil the effect was not reversed by the addition of calcium to the medium .
	manualset3
202622	5	417520	7	NULL	NULL	0	NULL	calcium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When beating ceased due to verapamil the effect was not reversed by the addition of calcium to the medium .
	manualset3
202623	6	417520	7	NULL	NULL	0	NULL	medium	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	When beating ceased due to verapamil the effect was not reversed by the addition of calcium to the medium .
	manualset3
202624	1	417521	7	NULL	NULL	0	NULL	bladder filling	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	When bladder filling was induced the median ureteric activity increased by 23 % in the non-refluxing ureters and by 25 % in refluxing ureters .
	manualset3
202625	2	417521	7	NULL	NULL	0	NULL	median ureteric activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When bladder filling was induced the median ureteric activity increased by 23 % in the non-refluxing ureters and by 25 % in refluxing ureters .
	manualset3
202626	3	417521	7	NULL	NULL	0	NULL	23 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When bladder filling was induced the median ureteric activity increased by 23 % in the non-refluxing ureters and by 25 % in refluxing ureters .
	manualset3
202627	4	417521	7	NULL	NULL	0	NULL	non-refluxing ureters	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	When bladder filling was induced the median ureteric activity increased by 23 % in the non-refluxing ureters and by 25 % in refluxing ureters .
	manualset3
202628	5	417521	7	NULL	NULL	0	NULL	25 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When bladder filling was induced the median ureteric activity increased by 23 % in the non-refluxing ureters and by 25 % in refluxing ureters .
	manualset3
202629	6	417521	7	NULL	NULL	0	NULL	refluxing ureters	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	When bladder filling was induced the median ureteric activity increased by 23 % in the non-refluxing ureters and by 25 % in refluxing ureters .
	manualset3
202630	1	417522	7	NULL	NULL	0	NULL	assessments 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When both assessments were compared , the concordance to assess relationship risk was 99.3 % .
	manualset3
202631	2	417522	7	NULL	NULL	0	NULL	 concordance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When both assessments were compared , the concordance to assess relationship risk was 99.3 % .
	manualset3
202632	3	417522	7	NULL	NULL	0	NULL	relationship risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When both assessments were compared , the concordance to assess relationship risk was 99.3 % .
	manualset3
202633	4	417522	7	NULL	NULL	0	NULL	99.3 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When both assessments were compared , the concordance to assess relationship risk was 99.3 % .
	manualset3
202634	1	417523	7	NULL	NULL	0	NULL	caterpillars	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When caterpillars fed on leaves of A. thaliana containing ( C ) - methylsulfinylbutyl glucosinolate , more than half of the ingested radioactivity was excreted as the unmetabolised corresponding isothiocyanate , and only 11 % as glutathione conjugate derivatives .
	manualset3
202635	2	417523	7	NULL	NULL	0	NULL	leaves	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When caterpillars fed on leaves of A. thaliana containing ( C ) - methylsulfinylbutyl glucosinolate , more than half of the ingested radioactivity was excreted as the unmetabolised corresponding isothiocyanate , and only 11 % as glutathione conjugate derivatives .
	manualset3
202636	3	417523	7	NULL	NULL	0	NULL	A. thaliana	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When caterpillars fed on leaves of A. thaliana containing ( C ) - methylsulfinylbutyl glucosinolate , more than half of the ingested radioactivity was excreted as the unmetabolised corresponding isothiocyanate , and only 11 % as glutathione conjugate derivatives .
	manualset3
202637	4	417523	7	NULL	NULL	0	NULL	 ( C ) - methylsulfinylbutyl glucosinolate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When caterpillars fed on leaves of A. thaliana containing ( C ) - methylsulfinylbutyl glucosinolate , more than half of the ingested radioactivity was excreted as the unmetabolised corresponding isothiocyanate , and only 11 % as glutathione conjugate derivatives .
	manualset3
202638	5	417523	7	NULL	NULL	0	NULL	half	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When caterpillars fed on leaves of A. thaliana containing ( C ) - methylsulfinylbutyl glucosinolate , more than half of the ingested radioactivity was excreted as the unmetabolised corresponding isothiocyanate , and only 11 % as glutathione conjugate derivatives .
	manualset3
202639	6	417523	7	NULL	NULL	NULL	NULL	ingested radioactivity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When caterpillars fed on leaves of A. thaliana containing ( C ) - methylsulfinylbutyl glucosinolate , more than half of the ingested radioactivity was excreted as the unmetabolised corresponding isothiocyanate , and only 11 % as glutathione conjugate derivatives .
	manualset3
202640	7	417523	7	NULL	NULL	0	NULL	isothiocyanate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When caterpillars fed on leaves of A. thaliana containing ( C ) - methylsulfinylbutyl glucosinolate , more than half of the ingested radioactivity was excreted as the unmetabolised corresponding isothiocyanate , and only 11 % as glutathione conjugate derivatives .
	manualset3
202641	8	417523	7	NULL	NULL	0	NULL	11 %	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When caterpillars fed on leaves of A. thaliana containing ( C ) - methylsulfinylbutyl glucosinolate , more than half of the ingested radioactivity was excreted as the unmetabolised corresponding isothiocyanate , and only 11 % as glutathione conjugate derivatives .
	manualset3
202642	9	417523	7	NULL	NULL	0	NULL	glutathione conjugate derivatives	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	When caterpillars fed on leaves of A. thaliana containing ( C ) - methylsulfinylbutyl glucosinolate , more than half of the ingested radioactivity was excreted as the unmetabolised corresponding isothiocyanate , and only 11 % as glutathione conjugate derivatives .
	manualset3
202643	1	417524	7	NULL	NULL	0	NULL	cell surface expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When cell surface expression of the alpha 1 subunit in 25 mM glucose was reduced , the alpha 2 subunit was involved in adhesion to a greater extent than it was in 5 mM glucose .
	manualset3
202644	2	417524	7	NULL	NULL	0	NULL	alpha 1 subunit	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When cell surface expression of the alpha 1 subunit in 25 mM glucose was reduced , the alpha 2 subunit was involved in adhesion to a greater extent than it was in 5 mM glucose .
	manualset3
202645	3	417524	7	NULL	NULL	0	NULL	25 mM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When cell surface expression of the alpha 1 subunit in 25 mM glucose was reduced , the alpha 2 subunit was involved in adhesion to a greater extent than it was in 5 mM glucose .
	manualset3
202646	4	417524	7	NULL	NULL	0	NULL	glucose	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When cell surface expression of the alpha 1 subunit in 25 mM glucose was reduced , the alpha 2 subunit was involved in adhesion to a greater extent than it was in 5 mM glucose .
	manualset3
202647	5	417524	7	NULL	NULL	0	NULL	alpha 2 subunit	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When cell surface expression of the alpha 1 subunit in 25 mM glucose was reduced , the alpha 2 subunit was involved in adhesion to a greater extent than it was in 5 mM glucose .
	manualset3
202648	6	417524	7	NULL	NULL	0	NULL	adhesion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When cell surface expression of the alpha 1 subunit in 25 mM glucose was reduced , the alpha 2 subunit was involved in adhesion to a greater extent than it was in 5 mM glucose .
	manualset3
202649	7	417524	7	NULL	NULL	0	NULL	5 mM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When cell surface expression of the alpha 1 subunit in 25 mM glucose was reduced , the alpha 2 subunit was involved in adhesion to a greater extent than it was in 5 mM glucose .
	manualset3
202650	8	417524	7	NULL	NULL	0	NULL	glucose	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When cell surface expression of the alpha 1 subunit in 25 mM glucose was reduced , the alpha 2 subunit was involved in adhesion to a greater extent than it was in 5 mM glucose .
	manualset3
202651	1	417525	7	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	When cells are stressed , a common response is to undergo cell death by one of two pathways , either ` necrosis ' or ` apoptosis ' .
	manualset3
202652	2	417525	7	NULL	NULL	0	NULL	 response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When cells are stressed , a common response is to undergo cell death by one of two pathways , either ` necrosis ' or ` apoptosis ' .
	manualset3
202653	3	417525	7	NULL	NULL	0	NULL	cell death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When cells are stressed , a common response is to undergo cell death by one of two pathways , either ` necrosis ' or ` apoptosis ' .
	manualset3
202654	4	417525	7	NULL	NULL	NULL	NULL	one pathway	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When cells are stressed , a common response is to undergo cell death by one of two pathways , either ` necrosis ' or ` apoptosis ' .
	manualset3
202655	5	417525	7	NULL	NULL	0	NULL	two pathways	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When cells are stressed , a common response is to undergo cell death by one of two pathways , either ` necrosis ' or ` apoptosis ' .
	manualset3
202656	6	417525	7	NULL	NULL	0	NULL	necrosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When cells are stressed , a common response is to undergo cell death by one of two pathways , either ` necrosis ' or ` apoptosis ' .
	manualset3
202657	7	417525	7	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When cells are stressed , a common response is to undergo cell death by one of two pathways , either ` necrosis ' or ` apoptosis ' .
	manualset3
202658	1	417526	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	When cells were incubated for 24 h and then continuously labeled for an additional 24 h , cellular conversion of labeled proinsulin to insulin was increased by glucose , and this increase was reversed or inhibited by 10 ( -6 ) M dexamethasone .
	manualset3
202659	2	417526	7	NULL	NULL	0	NULL	24 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	When cells were incubated for 24 h and then continuously labeled for an additional 24 h , cellular conversion of labeled proinsulin to insulin was increased by glucose , and this increase was reversed or inhibited by 10 ( -6 ) M dexamethasone .
	manualset3
202660	3	417526	7	NULL	NULL	0	NULL	24 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	When cells were incubated for 24 h and then continuously labeled for an additional 24 h , cellular conversion of labeled proinsulin to insulin was increased by glucose , and this increase was reversed or inhibited by 10 ( -6 ) M dexamethasone .
	manualset3
202661	4	417526	7	NULL	NULL	0	NULL	cellular conversion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When cells were incubated for 24 h and then continuously labeled for an additional 24 h , cellular conversion of labeled proinsulin to insulin was increased by glucose , and this increase was reversed or inhibited by 10 ( -6 ) M dexamethasone .
	manualset3
202662	5	417526	7	NULL	NULL	0	NULL	labeled proinsulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When cells were incubated for 24 h and then continuously labeled for an additional 24 h , cellular conversion of labeled proinsulin to insulin was increased by glucose , and this increase was reversed or inhibited by 10 ( -6 ) M dexamethasone .
	manualset3
202663	6	417526	7	NULL	NULL	0	NULL	 insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When cells were incubated for 24 h and then continuously labeled for an additional 24 h , cellular conversion of labeled proinsulin to insulin was increased by glucose , and this increase was reversed or inhibited by 10 ( -6 ) M dexamethasone .
	manualset3
202664	7	417526	7	NULL	NULL	NULL	NULL	 glucose	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When cells were incubated for 24 h and then continuously labeled for an additional 24 h , cellular conversion of labeled proinsulin to insulin was increased by glucose , and this increase was reversed or inhibited by 10 ( -6 ) M dexamethasone .
	manualset3
202665	8	417526	7	NULL	NULL	0	NULL	10 ( -6 ) M	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When cells were incubated for 24 h and then continuously labeled for an additional 24 h , cellular conversion of labeled proinsulin to insulin was increased by glucose , and this increase was reversed or inhibited by 10 ( -6 ) M dexamethasone .
	manualset3
202666	9	417526	7	NULL	NULL	0	NULL	dexamethasone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When cells were incubated for 24 h and then continuously labeled for an additional 24 h , cellular conversion of labeled proinsulin to insulin was increased by glucose , and this increase was reversed or inhibited by 10 ( -6 ) M dexamethasone .
	manualset3
204486	10	417526	7	NULL	NULL	NULL	NULL	increase	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When cells were incubated for 24 h and then continuously labeled for an additional 24 h , cellular conversion of labeled proinsulin to insulin was increased by glucose , and this increase was reversed or inhibited by 10 ( -6 ) M dexamethasone .
	manualset3
202667	1	417527	7	NULL	NULL	0	NULL	FAD-dependent halogenases	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When compared to the structurally known FAD-dependent halogenases PrnA and RebH , CndH lacks a 45 residue segment near position 100 and deviates in the C-terminal domain .
	manualset3
202668	2	417527	7	NULL	NULL	0	NULL	PrnA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When compared to the structurally known FAD-dependent halogenases PrnA and RebH , CndH lacks a 45 residue segment near position 100 and deviates in the C-terminal domain .
	manualset3
202669	3	417527	7	NULL	NULL	0	NULL	RebH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When compared to the structurally known FAD-dependent halogenases PrnA and RebH , CndH lacks a 45 residue segment near position 100 and deviates in the C-terminal domain .
	manualset3
202670	4	417527	7	NULL	NULL	0	NULL	CndH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When compared to the structurally known FAD-dependent halogenases PrnA and RebH , CndH lacks a 45 residue segment near position 100 and deviates in the C-terminal domain .
	manualset3
202671	5	417527	7	NULL	NULL	0	NULL	45 residue segment	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	When compared to the structurally known FAD-dependent halogenases PrnA and RebH , CndH lacks a 45 residue segment near position 100 and deviates in the C-terminal domain .
	manualset3
202672	6	417527	7	NULL	NULL	0	NULL	position 100	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	When compared to the structurally known FAD-dependent halogenases PrnA and RebH , CndH lacks a 45 residue segment near position 100 and deviates in the C-terminal domain .
	manualset3
202674	8	417527	7	NULL	NULL	0	NULL	C-terminal domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	When compared to the structurally known FAD-dependent halogenases PrnA and RebH , CndH lacks a 45 residue segment near position 100 and deviates in the C-terminal domain .
	manualset3
202675	1	417528	7	NULL	NULL	0	NULL	routine histologic sections	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	When compared with routine histologic sections stained with hematoxylin and eosin , blood vessels were much easier to identify in sections stained histochemically with DBA .
	manualset3
202676	2	417528	7	NULL	NULL	0	NULL	hematoxylin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When compared with routine histologic sections stained with hematoxylin and eosin , blood vessels were much easier to identify in sections stained histochemically with DBA .
	manualset3
202677	3	417528	7	NULL	NULL	0	NULL	eosin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When compared with routine histologic sections stained with hematoxylin and eosin , blood vessels were much easier to identify in sections stained histochemically with DBA .
	manualset3
202678	4	417528	7	NULL	NULL	0	NULL	blood vessels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When compared with routine histologic sections stained with hematoxylin and eosin , blood vessels were much easier to identify in sections stained histochemically with DBA .
	manualset3
202679	5	417528	7	NULL	NULL	NULL	NULL	sections	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When compared with routine histologic sections stained with hematoxylin and eosin , blood vessels were much easier to identify in sections stained histochemically with DBA .
	manualset3
202680	6	417528	7	NULL	NULL	0	NULL	DBA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When compared with routine histologic sections stained with hematoxylin and eosin , blood vessels were much easier to identify in sections stained histochemically with DBA .
	manualset3
202692	1	417529	7	NULL	NULL	NULL	NULL	prognostic patients ' characteristics	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When comparing the prognostic patients ' characteristics , patients with 2677 GT genotype were statistically linked to the unmutated IgVH genes ( r = 0.209 , P = 0.01 ) .
	manualset3
202693	2	417529	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When comparing the prognostic patients ' characteristics , patients with 2677 GT genotype were statistically linked to the unmutated IgVH genes ( r = 0.209 , P = 0.01 ) .
	manualset3
202694	3	417529	7	NULL	NULL	0	NULL	2677 GT genotype	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	When comparing the prognostic patients ' characteristics , patients with 2677 GT genotype were statistically linked to the unmutated IgVH genes ( r = 0.209 , P = 0.01 ) .
	manualset3
202695	4	417529	7	NULL	NULL	0	NULL	unmutated IgVH genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When comparing the prognostic patients ' characteristics , patients with 2677 GT genotype were statistically linked to the unmutated IgVH genes ( r = 0.209 , P = 0.01 ) .
	manualset3
202696	5	417529	7	NULL	NULL	0	NULL	 r = 0.209	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	When comparing the prognostic patients ' characteristics , patients with 2677 GT genotype were statistically linked to the unmutated IgVH genes ( r = 0.209 , P = 0.01 ) .
	manualset3
202697	6	417529	7	NULL	NULL	0	NULL	P = 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	When comparing the prognostic patients ' characteristics , patients with 2677 GT genotype were statistically linked to the unmutated IgVH genes ( r = 0.209 , P = 0.01 ) .
	manualset3
202712	1	417530	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When considering patients in an acute episode ( 52 % depressed ) , the CDSS score was correlated only with the PANSS positive sub-scale score .
	manualset3
202716	2	417530	7	NULL	NULL	0	NULL	acute episode	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When considering patients in an acute episode ( 52 % depressed ) , the CDSS score was correlated only with the PANSS positive sub-scale score .
	manualset3
202718	3	417530	7	NULL	NULL	0	NULL	52 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When considering patients in an acute episode ( 52 % depressed ) , the CDSS score was correlated only with the PANSS positive sub-scale score .
	manualset3
202719	4	417530	7	NULL	NULL	0	NULL	 CDSS score	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When considering patients in an acute episode ( 52 % depressed ) , the CDSS score was correlated only with the PANSS positive sub-scale score .
	manualset3
202720	5	417530	7	NULL	NULL	0	NULL	PANSS positive sub-scale score	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When considering patients in an acute episode ( 52 % depressed ) , the CDSS score was correlated only with the PANSS positive sub-scale score .
	manualset3
203015	1	417531	7	NULL	NULL	0	NULL	lower value 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When considering the lower value of umbilical vein pH at birth to be 7.20 , and the normal value of SPO2 during labor to be ) or = 40 % ( negative test ) , we observed a 100 % negative predictive value of oximetry .
	manualset3
203016	2	417531	7	NULL	NULL	0	NULL	umbilical vein pH 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When considering the lower value of umbilical vein pH at birth to be 7.20 , and the normal value of SPO2 during labor to be ) or = 40 % ( negative test ) , we observed a 100 % negative predictive value of oximetry .
	manualset3
203017	3	417531	7	NULL	NULL	0	NULL	birth 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When considering the lower value of umbilical vein pH at birth to be 7.20 , and the normal value of SPO2 during labor to be ) or = 40 % ( negative test ) , we observed a 100 % negative predictive value of oximetry .
	manualset3
203018	4	417531	7	NULL	NULL	0	NULL	7.20	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	When considering the lower value of umbilical vein pH at birth to be 7.20 , and the normal value of SPO2 during labor to be ) or = 40 % ( negative test ) , we observed a 100 % negative predictive value of oximetry .
	manualset3
203019	5	417531	7	NULL	NULL	0	NULL	normal value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When considering the lower value of umbilical vein pH at birth to be 7.20 , and the normal value of SPO2 during labor to be ) or = 40 % ( negative test ) , we observed a 100 % negative predictive value of oximetry .
	manualset3
203020	6	417531	7	NULL	NULL	0	NULL	SPO2	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When considering the lower value of umbilical vein pH at birth to be 7.20 , and the normal value of SPO2 during labor to be ) or = 40 % ( negative test ) , we observed a 100 % negative predictive value of oximetry .
	manualset3
203021	7	417531	7	NULL	NULL	0	NULL	labor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When considering the lower value of umbilical vein pH at birth to be 7.20 , and the normal value of SPO2 during labor to be ) or = 40 % ( negative test ) , we observed a 100 % negative predictive value of oximetry .
	manualset3
203022	8	417531	7	NULL	NULL	0	NULL	 40 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When considering the lower value of umbilical vein pH at birth to be 7.20 , and the normal value of SPO2 during labor to be ) or = 40 % ( negative test ) , we observed a 100 % negative predictive value of oximetry .
	manualset3
203023	9	417531	7	NULL	NULL	0	NULL	negative test	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	When considering the lower value of umbilical vein pH at birth to be 7.20 , and the normal value of SPO2 during labor to be ) or = 40 % ( negative test ) , we observed a 100 % negative predictive value of oximetry .
	manualset3
203024	10	417531	7	NULL	NULL	0	NULL	100 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When considering the lower value of umbilical vein pH at birth to be 7.20 , and the normal value of SPO2 during labor to be ) or = 40 % ( negative test ) , we observed a 100 % negative predictive value of oximetry .
	manualset3
203025	11	417531	7	NULL	NULL	0	NULL	negative predictive value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When considering the lower value of umbilical vein pH at birth to be 7.20 , and the normal value of SPO2 during labor to be ) or = 40 % ( negative test ) , we observed a 100 % negative predictive value of oximetry .
	manualset3
203026	12	417531	7	NULL	NULL	0	NULL	oximetry	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	When considering the lower value of umbilical vein pH at birth to be 7.20 , and the normal value of SPO2 during labor to be ) or = 40 % ( negative test ) , we observed a 100 % negative predictive value of oximetry .
	manualset3
203027	1	417532	7	NULL	NULL	0	NULL	coughing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When coughing can cause stroke -- a case-based update on cerebral air embolism complicating biopsy of the lung .
	manualset3
203028	2	417532	7	NULL	NULL	0	NULL	 stroke	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When coughing can cause stroke -- a case-based update on cerebral air embolism complicating biopsy of the lung .
	manualset3
203029	3	417532	7	NULL	NULL	0	NULL	case-based update	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	When coughing can cause stroke -- a case-based update on cerebral air embolism complicating biopsy of the lung .
	manualset3
203030	4	417532	7	NULL	NULL	0	NULL	cerebral air embolism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When coughing can cause stroke -- a case-based update on cerebral air embolism complicating biopsy of the lung .
	manualset3
203031	5	417532	7	NULL	NULL	0	NULL	biopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	When coughing can cause stroke -- a case-based update on cerebral air embolism complicating biopsy of the lung .
	manualset3
203032	6	417532	7	NULL	NULL	0	NULL	 lung	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When coughing can cause stroke -- a case-based update on cerebral air embolism complicating biopsy of the lung .
	manualset3
203098	1	417533	7	NULL	NULL	0	NULL	employees	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When dangerous employees cause harm .
	manualset3
203099	1	417534	7	NULL	NULL	0	NULL	dissolution experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	When dissolution experiments were complete , the aquifer model was excavated , and the distribution of NAPL zones was recorded using digital images of excavation grids .
	manualset3
203100	2	417534	7	NULL	NULL	0	NULL	aquifer model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	When dissolution experiments were complete , the aquifer model was excavated , and the distribution of NAPL zones was recorded using digital images of excavation grids .
	manualset3
203101	3	417534	7	NULL	NULL	0	NULL	 distribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When dissolution experiments were complete , the aquifer model was excavated , and the distribution of NAPL zones was recorded using digital images of excavation grids .
	manualset3
203102	4	417534	7	NULL	NULL	0	NULL	NAPL zones	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When dissolution experiments were complete , the aquifer model was excavated , and the distribution of NAPL zones was recorded using digital images of excavation grids .
	manualset3
203103	5	417534	7	NULL	NULL	0	NULL	digital images	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When dissolution experiments were complete , the aquifer model was excavated , and the distribution of NAPL zones was recorded using digital images of excavation grids .
	manualset3
203104	6	417534	7	NULL	NULL	NULL	NULL	excavation grids 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When dissolution experiments were complete , the aquifer model was excavated , and the distribution of NAPL zones was recorded using digital images of excavation grids .
	manualset3
203105	1	417535	7	NULL	NULL	0	NULL	monosaccharides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All monosaccharides , purines , pyrimidines , and nucleosides tested failed to induce germination of T. mentagrophytes arthrospores .
	manualset3
203106	2	417535	7	NULL	NULL	0	NULL	purines	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All monosaccharides , purines , pyrimidines , and nucleosides tested failed to induce germination of T. mentagrophytes arthrospores .
	manualset3
203107	3	417535	7	NULL	NULL	0	NULL	pyrimidines	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All monosaccharides , purines , pyrimidines , and nucleosides tested failed to induce germination of T. mentagrophytes arthrospores .
	manualset3
203108	4	417535	7	NULL	NULL	0	NULL	nucleosides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All monosaccharides , purines , pyrimidines , and nucleosides tested failed to induce germination of T. mentagrophytes arthrospores .
	manualset3
203109	5	417535	7	NULL	NULL	0	NULL	 germination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All monosaccharides , purines , pyrimidines , and nucleosides tested failed to induce germination of T. mentagrophytes arthrospores .
	manualset3
203110	6	417535	7	NULL	NULL	0	NULL	T. mentagrophytes arthrospores	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	All monosaccharides , purines , pyrimidines , and nucleosides tested failed to induce germination of T. mentagrophytes arthrospores .
	manualset3
203126	1	417537	7	NULL	NULL	0	NULL	estrogen	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When estrogen is reduced in the body , local factors such as IL-1beta and IL-6 , which are known to be related with bone resorption , are increased and promote osteoclastogenesis , which is responsible for bone resorption .
	manualset3
203127	2	417537	7	NULL	NULL	0	NULL	body	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When estrogen is reduced in the body , local factors such as IL-1beta and IL-6 , which are known to be related with bone resorption , are increased and promote osteoclastogenesis , which is responsible for bone resorption .
	manualset3
203128	3	417537	7	NULL	NULL	0	NULL	local factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When estrogen is reduced in the body , local factors such as IL-1beta and IL-6 , which are known to be related with bone resorption , are increased and promote osteoclastogenesis , which is responsible for bone resorption .
	manualset3
203129	4	417537	7	NULL	NULL	0	NULL	IL-1beta	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When estrogen is reduced in the body , local factors such as IL-1beta and IL-6 , which are known to be related with bone resorption , are increased and promote osteoclastogenesis , which is responsible for bone resorption .
	manualset3
203130	5	417537	7	NULL	NULL	0	NULL	IL-6	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When estrogen is reduced in the body , local factors such as IL-1beta and IL-6 , which are known to be related with bone resorption , are increased and promote osteoclastogenesis , which is responsible for bone resorption .
	manualset3
203131	6	417537	7	NULL	NULL	0	NULL	bone resorption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When estrogen is reduced in the body , local factors such as IL-1beta and IL-6 , which are known to be related with bone resorption , are increased and promote osteoclastogenesis , which is responsible for bone resorption .
	manualset3
203132	7	417537	7	NULL	NULL	0	NULL	osteoclastogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When estrogen is reduced in the body , local factors such as IL-1beta and IL-6 , which are known to be related with bone resorption , are increased and promote osteoclastogenesis , which is responsible for bone resorption .
	manualset3
203133	8	417537	7	NULL	NULL	0	NULL	bone resorption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When estrogen is reduced in the body , local factors such as IL-1beta and IL-6 , which are known to be related with bone resorption , are increased and promote osteoclastogenesis , which is responsible for bone resorption .
	manualset3
203134	1	417538	7	NULL	NULL	NULL	NULL	exogenous human estrogen receptor  ( hER ) 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When exogenous human estrogen receptor ( hER ) binds with estrogen , it can activate transcription of target genes in yeast cells .
	manualset3
203135	2	417538	7	NULL	NULL	0	NULL	estrogen	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When exogenous human estrogen receptor ( hER ) binds with estrogen , it can activate transcription of target genes in yeast cells .
	manualset3
203136	3	417538	7	NULL	NULL	0	NULL	transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When exogenous human estrogen receptor ( hER ) binds with estrogen , it can activate transcription of target genes in yeast cells .
	manualset3
203137	4	417538	7	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When exogenous human estrogen receptor ( hER ) binds with estrogen , it can activate transcription of target genes in yeast cells .
	manualset3
203138	5	417538	7	NULL	NULL	0	NULL	yeast cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	When exogenous human estrogen receptor ( hER ) binds with estrogen , it can activate transcription of target genes in yeast cells .
	manualset3
203139	1	417539	7	NULL	NULL	0	NULL	Xenopus oocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	When expressed alone in Xenopus oocytes , wild type connexin37 produced hemichannel currents , but neither of the double substitution mutants produced detectable currents .
	manualset3
203140	2	417539	7	NULL	NULL	0	NULL	wild type	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When expressed alone in Xenopus oocytes , wild type connexin37 produced hemichannel currents , but neither of the double substitution mutants produced detectable currents .
	manualset3
203141	3	417539	7	NULL	NULL	0	NULL	connexin37 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When expressed alone in Xenopus oocytes , wild type connexin37 produced hemichannel currents , but neither of the double substitution mutants produced detectable currents .
	manualset3
203142	4	417539	7	NULL	NULL	NULL	NULL	hemichannel currents	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When expressed alone in Xenopus oocytes , wild type connexin37 produced hemichannel currents , but neither of the double substitution mutants produced detectable currents .
	manualset3
203143	5	417539	7	NULL	NULL	0	NULL	 double substitution mutants	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When expressed alone in Xenopus oocytes , wild type connexin37 produced hemichannel currents , but neither of the double substitution mutants produced detectable currents .
	manualset3
203144	6	417539	7	NULL	NULL	NULL	NULL	currents	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When expressed alone in Xenopus oocytes , wild type connexin37 produced hemichannel currents , but neither of the double substitution mutants produced detectable currents .
	manualset3
203145	1	417540	7	NULL	NULL	0	NULL	 eye	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When eye creates the contact !
	manualset3
203146	2	417540	7	NULL	NULL	0	NULL	contact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When eye creates the contact !
	manualset3
203232	1	417541	7	NULL	NULL	0	NULL	 findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When findings for 805 patients followed at the two clinics were combined , 61 % met the CDC criteria , 55 % met the British criteria , and 56 % met the Australian criteria ; these proportions were relatively similar at both sites .
	manualset3
203233	2	417541	7	NULL	NULL	0	NULL	 805 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When findings for 805 patients followed at the two clinics were combined , 61 % met the CDC criteria , 55 % met the British criteria , and 56 % met the Australian criteria ; these proportions were relatively similar at both sites .
	manualset3
203234	3	417541	7	NULL	NULL	0	NULL	two clinics	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	When findings for 805 patients followed at the two clinics were combined , 61 % met the CDC criteria , 55 % met the British criteria , and 56 % met the Australian criteria ; these proportions were relatively similar at both sites .
	manualset3
203235	4	417541	7	NULL	NULL	0	NULL	 61 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When findings for 805 patients followed at the two clinics were combined , 61 % met the CDC criteria , 55 % met the British criteria , and 56 % met the Australian criteria ; these proportions were relatively similar at both sites .
	manualset3
203236	5	417541	7	NULL	NULL	0	NULL	CDC criteria	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When findings for 805 patients followed at the two clinics were combined , 61 % met the CDC criteria , 55 % met the British criteria , and 56 % met the Australian criteria ; these proportions were relatively similar at both sites .
	manualset3
203237	6	417541	7	NULL	NULL	0	NULL	55 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When findings for 805 patients followed at the two clinics were combined , 61 % met the CDC criteria , 55 % met the British criteria , and 56 % met the Australian criteria ; these proportions were relatively similar at both sites .
	manualset3
203238	7	417541	7	NULL	NULL	0	NULL	British criteria	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When findings for 805 patients followed at the two clinics were combined , 61 % met the CDC criteria , 55 % met the British criteria , and 56 % met the Australian criteria ; these proportions were relatively similar at both sites .
	manualset3
203239	8	417541	7	NULL	NULL	0	NULL	56 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When findings for 805 patients followed at the two clinics were combined , 61 % met the CDC criteria , 55 % met the British criteria , and 56 % met the Australian criteria ; these proportions were relatively similar at both sites .
	manualset3
203240	9	417541	7	NULL	NULL	0	NULL	Australian criteria	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When findings for 805 patients followed at the two clinics were combined , 61 % met the CDC criteria , 55 % met the British criteria , and 56 % met the Australian criteria ; these proportions were relatively similar at both sites .
	manualset3
203241	10	417541	7	NULL	NULL	0	NULL	proportions 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When findings for 805 patients followed at the two clinics were combined , 61 % met the CDC criteria , 55 % met the British criteria , and 56 % met the Australian criteria ; these proportions were relatively similar at both sites .
	manualset3
203242	11	417541	7	NULL	NULL	0	NULL	 sites	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	When findings for 805 patients followed at the two clinics were combined , 61 % met the CDC criteria , 55 % met the British criteria , and 56 % met the Australian criteria ; these proportions were relatively similar at both sites .
	manualset3
203244	2	417542	7	NULL	NULL	0	NULL	management plan	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When formulating a management plan for the elite athlete , the physician must consider `` doping '' rules and the possible effect of medication on athletic performance .
	manualset3
203245	3	417542	7	NULL	NULL	0	NULL	 elite athlete	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	When formulating a management plan for the elite athlete , the physician must consider `` doping '' rules and the possible effect of medication on athletic performance .
	manualset3
203246	4	417542	7	NULL	NULL	0	NULL	 physician	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	When formulating a management plan for the elite athlete , the physician must consider `` doping '' rules and the possible effect of medication on athletic performance .
	manualset3
203247	5	417542	7	NULL	NULL	0	NULL	`` doping '' rules 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When formulating a management plan for the elite athlete , the physician must consider `` doping '' rules and the possible effect of medication on athletic performance .
	manualset3
203248	6	417542	7	NULL	NULL	0	NULL	 medication	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	When formulating a management plan for the elite athlete , the physician must consider `` doping '' rules and the possible effect of medication on athletic performance .
	manualset3
203249	7	417542	7	NULL	NULL	0	NULL	athletic performance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When formulating a management plan for the elite athlete , the physician must consider `` doping '' rules and the possible effect of medication on athletic performance .
	manualset3
205489	8	417542	7	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When formulating a management plan for the elite athlete , the physician must consider `` doping '' rules and the possible effect of medication on athletic performance .
	manualset3
203250	1	417543	7	NULL	NULL	0	NULL	 genetic factors	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	When genetic factors are identical , obesity is associated with an atherogenic lipid profile , especially in subjects with high visceral fat accumulation .
	manualset3
203251	2	417543	7	NULL	NULL	0	NULL	obesity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When genetic factors are identical , obesity is associated with an atherogenic lipid profile , especially in subjects with high visceral fat accumulation .
	manualset3
203252	3	417543	7	NULL	NULL	NULL	NULL	atherogenic lipid profile	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When genetic factors are identical , obesity is associated with an atherogenic lipid profile , especially in subjects with high visceral fat accumulation .
	manualset3
203253	4	417543	7	NULL	NULL	0	NULL	subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When genetic factors are identical , obesity is associated with an atherogenic lipid profile , especially in subjects with high visceral fat accumulation .
	manualset3
203254	5	417543	7	NULL	NULL	0	NULL	high visceral fat accumulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When genetic factors are identical , obesity is associated with an atherogenic lipid profile , especially in subjects with high visceral fat accumulation .
	manualset3
203255	1	417544	7	NULL	NULL	0	NULL	rat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When given orally to a rat , CPCA-carnitine is excreted readily in urine as free CPCA and its glycine conjugate .
	manualset3
203256	2	417544	7	NULL	NULL	0	NULL	CPCA-carnitine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When given orally to a rat , CPCA-carnitine is excreted readily in urine as free CPCA and its glycine conjugate .
	manualset3
203257	3	417544	7	NULL	NULL	0	NULL	urine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When given orally to a rat , CPCA-carnitine is excreted readily in urine as free CPCA and its glycine conjugate .
	manualset3
203258	4	417544	7	NULL	NULL	0	NULL	free CPCA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When given orally to a rat , CPCA-carnitine is excreted readily in urine as free CPCA and its glycine conjugate .
	manualset3
203259	5	417544	7	NULL	NULL	0	NULL	glycine conjugate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When given orally to a rat , CPCA-carnitine is excreted readily in urine as free CPCA and its glycine conjugate .
	manualset3
203260	1	417545	7	NULL	NULL	0	NULL	operations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All operations had been performed by the same surgeon using the same design of prosthesis at a single institution .
	manualset3
203261	2	417545	7	NULL	NULL	0	NULL	surgeon	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	All operations had been performed by the same surgeon using the same design of prosthesis at a single institution .
	manualset3
203262	3	417545	7	NULL	NULL	0	NULL	 design	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	All operations had been performed by the same surgeon using the same design of prosthesis at a single institution .
	manualset3
203263	4	417545	7	NULL	NULL	0	NULL	prosthesis	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	All operations had been performed by the same surgeon using the same design of prosthesis at a single institution .
	manualset3
203264	5	417545	7	NULL	NULL	0	NULL	single institution	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	All operations had been performed by the same surgeon using the same design of prosthesis at a single institution .
	manualset3
203265	1	417546	7	NULL	NULL	0	NULL	grafts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When grafts with thromboses were compared to those without thrombosis by univariate analysis , access blood flow measured either by ultrasound dilution technique ( 875 + / - 426 ml/min with thrombosis vs. 1193 + / - 677 ml/min without thrombosis , P = 0.001 ) or by Doppler ultrasound ( 762 + / - 420 ml/min with thrombosis vs. 1171 + / - 657 ml/min without thrombosis , P = 0.001 ) were significantly different in the two groups .
	manualset3
203266	2	417546	7	NULL	NULL	0	NULL	thromboses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When grafts with thromboses were compared to those without thrombosis by univariate analysis , access blood flow measured either by ultrasound dilution technique ( 875 + / - 426 ml/min with thrombosis vs. 1193 + / - 677 ml/min without thrombosis , P = 0.001 ) or by Doppler ultrasound ( 762 + / - 420 ml/min with thrombosis vs. 1171 + / - 657 ml/min without thrombosis , P = 0.001 ) were significantly different in the two groups .
	manualset3
203267	3	417546	7	NULL	NULL	0	NULL	thrombosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When grafts with thromboses were compared to those without thrombosis by univariate analysis , access blood flow measured either by ultrasound dilution technique ( 875 + / - 426 ml/min with thrombosis vs. 1193 + / - 677 ml/min without thrombosis , P = 0.001 ) or by Doppler ultrasound ( 762 + / - 420 ml/min with thrombosis vs. 1171 + / - 657 ml/min without thrombosis , P = 0.001 ) were significantly different in the two groups .
	manualset3
203268	4	417546	7	NULL	NULL	0	NULL	univariate analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	When grafts with thromboses were compared to those without thrombosis by univariate analysis , access blood flow measured either by ultrasound dilution technique ( 875 + / - 426 ml/min with thrombosis vs. 1193 + / - 677 ml/min without thrombosis , P = 0.001 ) or by Doppler ultrasound ( 762 + / - 420 ml/min with thrombosis vs. 1171 + / - 657 ml/min without thrombosis , P = 0.001 ) were significantly different in the two groups .
	manualset3
203269	5	417546	7	NULL	NULL	0	NULL	blood flow	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When grafts with thromboses were compared to those without thrombosis by univariate analysis , access blood flow measured either by ultrasound dilution technique ( 875 + / - 426 ml/min with thrombosis vs. 1193 + / - 677 ml/min without thrombosis , P = 0.001 ) or by Doppler ultrasound ( 762 + / - 420 ml/min with thrombosis vs. 1171 + / - 657 ml/min without thrombosis , P = 0.001 ) were significantly different in the two groups .
	manualset3
203270	6	417546	7	NULL	NULL	0	NULL	 ultrasound dilution technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	When grafts with thromboses were compared to those without thrombosis by univariate analysis , access blood flow measured either by ultrasound dilution technique ( 875 + / - 426 ml/min with thrombosis vs. 1193 + / - 677 ml/min without thrombosis , P = 0.001 ) or by Doppler ultrasound ( 762 + / - 420 ml/min with thrombosis vs. 1171 + / - 657 ml/min without thrombosis , P = 0.001 ) were significantly different in the two groups .
	manualset3
203272	7	417546	7	NULL	NULL	0	NULL	 875 + / - 426 ml/min 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	When grafts with thromboses were compared to those without thrombosis by univariate analysis , access blood flow measured either by ultrasound dilution technique ( 875 + / - 426 ml/min with thrombosis vs. 1193 + / - 677 ml/min without thrombosis , P = 0.001 ) or by Doppler ultrasound ( 762 + / - 420 ml/min with thrombosis vs. 1171 + / - 657 ml/min without thrombosis , P = 0.001 ) were significantly different in the two groups .
	manualset3
203273	8	417546	7	NULL	NULL	0	NULL	thrombosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When grafts with thromboses were compared to those without thrombosis by univariate analysis , access blood flow measured either by ultrasound dilution technique ( 875 + / - 426 ml/min with thrombosis vs. 1193 + / - 677 ml/min without thrombosis , P = 0.001 ) or by Doppler ultrasound ( 762 + / - 420 ml/min with thrombosis vs. 1171 + / - 657 ml/min without thrombosis , P = 0.001 ) were significantly different in the two groups .
	manualset3
203275	9	417546	7	NULL	NULL	0	NULL	1193 + / - 677 ml/min	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	When grafts with thromboses were compared to those without thrombosis by univariate analysis , access blood flow measured either by ultrasound dilution technique ( 875 + / - 426 ml/min with thrombosis vs. 1193 + / - 677 ml/min without thrombosis , P = 0.001 ) or by Doppler ultrasound ( 762 + / - 420 ml/min with thrombosis vs. 1171 + / - 657 ml/min without thrombosis , P = 0.001 ) were significantly different in the two groups .
	manualset3
203277	10	417546	7	NULL	NULL	0	NULL	thrombosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When grafts with thromboses were compared to those without thrombosis by univariate analysis , access blood flow measured either by ultrasound dilution technique ( 875 + / - 426 ml/min with thrombosis vs. 1193 + / - 677 ml/min without thrombosis , P = 0.001 ) or by Doppler ultrasound ( 762 + / - 420 ml/min with thrombosis vs. 1171 + / - 657 ml/min without thrombosis , P = 0.001 ) were significantly different in the two groups .
	manualset3
203281	11	417546	7	NULL	NULL	0	NULL	P = 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	When grafts with thromboses were compared to those without thrombosis by univariate analysis , access blood flow measured either by ultrasound dilution technique ( 875 + / - 426 ml/min with thrombosis vs. 1193 + / - 677 ml/min without thrombosis , P = 0.001 ) or by Doppler ultrasound ( 762 + / - 420 ml/min with thrombosis vs. 1171 + / - 657 ml/min without thrombosis , P = 0.001 ) were significantly different in the two groups .
	manualset3
203282	12	417546	7	NULL	NULL	0	NULL	Doppler ultrasound	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	When grafts with thromboses were compared to those without thrombosis by univariate analysis , access blood flow measured either by ultrasound dilution technique ( 875 + / - 426 ml/min with thrombosis vs. 1193 + / - 677 ml/min without thrombosis , P = 0.001 ) or by Doppler ultrasound ( 762 + / - 420 ml/min with thrombosis vs. 1171 + / - 657 ml/min without thrombosis , P = 0.001 ) were significantly different in the two groups .
	manualset3
203283	13	417546	7	NULL	NULL	0	NULL	762 + / - 420 ml/min	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	When grafts with thromboses were compared to those without thrombosis by univariate analysis , access blood flow measured either by ultrasound dilution technique ( 875 + / - 426 ml/min with thrombosis vs. 1193 + / - 677 ml/min without thrombosis , P = 0.001 ) or by Doppler ultrasound ( 762 + / - 420 ml/min with thrombosis vs. 1171 + / - 657 ml/min without thrombosis , P = 0.001 ) were significantly different in the two groups .
	manualset3
203284	14	417546	7	NULL	NULL	NULL	NULL	thrombosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When grafts with thromboses were compared to those without thrombosis by univariate analysis , access blood flow measured either by ultrasound dilution technique ( 875 + / - 426 ml/min with thrombosis vs. 1193 + / - 677 ml/min without thrombosis , P = 0.001 ) or by Doppler ultrasound ( 762 + / - 420 ml/min with thrombosis vs. 1171 + / - 657 ml/min without thrombosis , P = 0.001 ) were significantly different in the two groups .
	manualset3
203285	15	417546	7	NULL	NULL	0	NULL	1171 + / - 657 ml/min 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	When grafts with thromboses were compared to those without thrombosis by univariate analysis , access blood flow measured either by ultrasound dilution technique ( 875 + / - 426 ml/min with thrombosis vs. 1193 + / - 677 ml/min without thrombosis , P = 0.001 ) or by Doppler ultrasound ( 762 + / - 420 ml/min with thrombosis vs. 1171 + / - 657 ml/min without thrombosis , P = 0.001 ) were significantly different in the two groups .
	manualset3
203286	16	417546	7	NULL	NULL	0	NULL	thrombosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When grafts with thromboses were compared to those without thrombosis by univariate analysis , access blood flow measured either by ultrasound dilution technique ( 875 + / - 426 ml/min with thrombosis vs. 1193 + / - 677 ml/min without thrombosis , P = 0.001 ) or by Doppler ultrasound ( 762 + / - 420 ml/min with thrombosis vs. 1171 + / - 657 ml/min without thrombosis , P = 0.001 ) were significantly different in the two groups .
	manualset3
203287	17	417546	7	NULL	NULL	0	NULL	P = 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	When grafts with thromboses were compared to those without thrombosis by univariate analysis , access blood flow measured either by ultrasound dilution technique ( 875 + / - 426 ml/min with thrombosis vs. 1193 + / - 677 ml/min without thrombosis , P = 0.001 ) or by Doppler ultrasound ( 762 + / - 420 ml/min with thrombosis vs. 1171 + / - 657 ml/min without thrombosis , P = 0.001 ) were significantly different in the two groups .
	manualset3
203288	18	417546	7	NULL	NULL	0	NULL	two groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When grafts with thromboses were compared to those without thrombosis by univariate analysis , access blood flow measured either by ultrasound dilution technique ( 875 + / - 426 ml/min with thrombosis vs. 1193 + / - 677 ml/min without thrombosis , P = 0.001 ) or by Doppler ultrasound ( 762 + / - 420 ml/min with thrombosis vs. 1171 + / - 657 ml/min without thrombosis , P = 0.001 ) were significantly different in the two groups .
	manualset3
203295	1	417547	7	NULL	NULL	0	NULL	media	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	When grown in rich media , single-celled organisms such as yeast and bacteria can be up to twice the size of their slow-growing counterparts .
	manualset3
203302	2	417547	7	NULL	NULL	0	NULL	single-celled organisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When grown in rich media , single-celled organisms such as yeast and bacteria can be up to twice the size of their slow-growing counterparts .
	manualset3
203304	3	417547	7	NULL	NULL	0	NULL	yeast	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When grown in rich media , single-celled organisms such as yeast and bacteria can be up to twice the size of their slow-growing counterparts .
	manualset3
203305	4	417547	7	NULL	NULL	0	NULL	bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When grown in rich media , single-celled organisms such as yeast and bacteria can be up to twice the size of their slow-growing counterparts .
	manualset3
203307	5	417547	7	NULL	NULL	0	NULL	 size 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When grown in rich media , single-celled organisms such as yeast and bacteria can be up to twice the size of their slow-growing counterparts .
	manualset3
203324	6	417547	7	NULL	NULL	0	NULL	slow-growing counterparts	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When grown in rich media , single-celled organisms such as yeast and bacteria can be up to twice the size of their slow-growing counterparts .
	manualset3
203326	7	417547	7	NULL	NULL	0	NULL	twice	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When grown in rich media , single-celled organisms such as yeast and bacteria can be up to twice the size of their slow-growing counterparts .
	manualset3
203329	1	417548	7	NULL	NULL	0	NULL	guinea-pig hearts 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When guinea-pig hearts were perfused with 3 X 10 ( -6 ) M denopamine or 10 ( -7 ) M isoproterenol , their cardiotonic effects were of the same magnitude whereas the degree of c-AMP elevation in the ventricular tissue by denopamine was significantly less than that by isoproterenol .
	manualset3
203331	2	417548	7	NULL	NULL	0	NULL	3 X 10 ( -6 ) M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	When guinea-pig hearts were perfused with 3 X 10 ( -6 ) M denopamine or 10 ( -7 ) M isoproterenol , their cardiotonic effects were of the same magnitude whereas the degree of c-AMP elevation in the ventricular tissue by denopamine was significantly less than that by isoproterenol .
	manualset3
203332	3	417548	7	NULL	NULL	0	NULL	denopamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When guinea-pig hearts were perfused with 3 X 10 ( -6 ) M denopamine or 10 ( -7 ) M isoproterenol , their cardiotonic effects were of the same magnitude whereas the degree of c-AMP elevation in the ventricular tissue by denopamine was significantly less than that by isoproterenol .
	manualset3
203333	4	417548	7	NULL	NULL	NULL	NULL	10 ( -7 ) M	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When guinea-pig hearts were perfused with 3 X 10 ( -6 ) M denopamine or 10 ( -7 ) M isoproterenol , their cardiotonic effects were of the same magnitude whereas the degree of c-AMP elevation in the ventricular tissue by denopamine was significantly less than that by isoproterenol .
	manualset3
203334	5	417548	7	NULL	NULL	0	NULL	isoproterenol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When guinea-pig hearts were perfused with 3 X 10 ( -6 ) M denopamine or 10 ( -7 ) M isoproterenol , their cardiotonic effects were of the same magnitude whereas the degree of c-AMP elevation in the ventricular tissue by denopamine was significantly less than that by isoproterenol .
	manualset3
203335	6	417548	7	NULL	NULL	0	NULL	cardiotonic effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When guinea-pig hearts were perfused with 3 X 10 ( -6 ) M denopamine or 10 ( -7 ) M isoproterenol , their cardiotonic effects were of the same magnitude whereas the degree of c-AMP elevation in the ventricular tissue by denopamine was significantly less than that by isoproterenol .
	manualset3
203336	7	417548	7	NULL	NULL	0	NULL	magnitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When guinea-pig hearts were perfused with 3 X 10 ( -6 ) M denopamine or 10 ( -7 ) M isoproterenol , their cardiotonic effects were of the same magnitude whereas the degree of c-AMP elevation in the ventricular tissue by denopamine was significantly less than that by isoproterenol .
	manualset3
203337	8	417548	7	NULL	NULL	0	NULL	degree	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When guinea-pig hearts were perfused with 3 X 10 ( -6 ) M denopamine or 10 ( -7 ) M isoproterenol , their cardiotonic effects were of the same magnitude whereas the degree of c-AMP elevation in the ventricular tissue by denopamine was significantly less than that by isoproterenol .
	manualset3
203338	9	417548	7	NULL	NULL	0	NULL	c-AMP elevation	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When guinea-pig hearts were perfused with 3 X 10 ( -6 ) M denopamine or 10 ( -7 ) M isoproterenol , their cardiotonic effects were of the same magnitude whereas the degree of c-AMP elevation in the ventricular tissue by denopamine was significantly less than that by isoproterenol .
	manualset3
203339	10	417548	7	NULL	NULL	0	NULL	 ventricular tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	When guinea-pig hearts were perfused with 3 X 10 ( -6 ) M denopamine or 10 ( -7 ) M isoproterenol , their cardiotonic effects were of the same magnitude whereas the degree of c-AMP elevation in the ventricular tissue by denopamine was significantly less than that by isoproterenol .
	manualset3
203340	11	417548	7	NULL	NULL	0	NULL	denopamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When guinea-pig hearts were perfused with 3 X 10 ( -6 ) M denopamine or 10 ( -7 ) M isoproterenol , their cardiotonic effects were of the same magnitude whereas the degree of c-AMP elevation in the ventricular tissue by denopamine was significantly less than that by isoproterenol .
	manualset3
203341	12	417548	7	NULL	NULL	0	NULL	 isoproterenol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When guinea-pig hearts were perfused with 3 X 10 ( -6 ) M denopamine or 10 ( -7 ) M isoproterenol , their cardiotonic effects were of the same magnitude whereas the degree of c-AMP elevation in the ventricular tissue by denopamine was significantly less than that by isoproterenol .
	manualset3
203342	1	417549	7	NULL	NULL	0	NULL	 recovery	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When h and n are allowed to vary , recovery and refractoriness result from the movement with subsequent disappearance of the threshold and excited points .
	manualset3
203343	2	417549	7	NULL	NULL	0	NULL	refractoriness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When h and n are allowed to vary , recovery and refractoriness result from the movement with subsequent disappearance of the threshold and excited points .
	manualset3
203346	3	417549	7	NULL	NULL	0	NULL	movement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When h and n are allowed to vary , recovery and refractoriness result from the movement with subsequent disappearance of the threshold and excited points .
	manualset3
203348	4	417549	7	NULL	NULL	0	NULL	threshold 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When h and n are allowed to vary , recovery and refractoriness result from the movement with subsequent disappearance of the threshold and excited points .
	manualset3
203352	5	417549	7	NULL	NULL	NULL	NULL	excited points	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When h and n are allowed to vary , recovery and refractoriness result from the movement with subsequent disappearance of the threshold and excited points .
	manualset3
203355	6	417549	7	NULL	NULL	0	NULL	h	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When h and n are allowed to vary , recovery and refractoriness result from the movement with subsequent disappearance of the threshold and excited points .
	manualset3
203356	7	417549	7	NULL	NULL	0	NULL	n	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When h and n are allowed to vary , recovery and refractoriness result from the movement with subsequent disappearance of the threshold and excited points .
	manualset3
203357	1	417550	7	NULL	NULL	0	NULL	homogenates	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When homogenates of hypothalami or anterior pituitary glands were incubated with ( 3H ) Testosterone in the presence of a 50-fold excess of testosterone-17 beta CA , the formation of labeled DHT was inhibited by more than 80 % .
	manualset3
203360	2	417550	7	NULL	NULL	0	NULL	hypothalami 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When homogenates of hypothalami or anterior pituitary glands were incubated with ( 3H ) Testosterone in the presence of a 50-fold excess of testosterone-17 beta CA , the formation of labeled DHT was inhibited by more than 80 % .
	manualset3
203362	3	417550	7	NULL	NULL	0	NULL	anterior pituitary glands	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When homogenates of hypothalami or anterior pituitary glands were incubated with ( 3H ) Testosterone in the presence of a 50-fold excess of testosterone-17 beta CA , the formation of labeled DHT was inhibited by more than 80 % .
	manualset3
203365	4	417550	7	NULL	NULL	0	NULL	( 3H ) Testosterone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When homogenates of hypothalami or anterior pituitary glands were incubated with ( 3H ) Testosterone in the presence of a 50-fold excess of testosterone-17 beta CA , the formation of labeled DHT was inhibited by more than 80 % .
	manualset3
203367	5	417550	7	NULL	NULL	0	NULL	50-fold excess	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When homogenates of hypothalami or anterior pituitary glands were incubated with ( 3H ) Testosterone in the presence of a 50-fold excess of testosterone-17 beta CA , the formation of labeled DHT was inhibited by more than 80 % .
	manualset3
203369	6	417550	7	NULL	NULL	0	NULL	testosterone-17 beta CA	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When homogenates of hypothalami or anterior pituitary glands were incubated with ( 3H ) Testosterone in the presence of a 50-fold excess of testosterone-17 beta CA , the formation of labeled DHT was inhibited by more than 80 % .
	manualset3
203372	7	417550	7	NULL	NULL	0	NULL	formation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When homogenates of hypothalami or anterior pituitary glands were incubated with ( 3H ) Testosterone in the presence of a 50-fold excess of testosterone-17 beta CA , the formation of labeled DHT was inhibited by more than 80 % .
	manualset3
203373	8	417550	7	NULL	NULL	0	NULL	labeled DHT	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When homogenates of hypothalami or anterior pituitary glands were incubated with ( 3H ) Testosterone in the presence of a 50-fold excess of testosterone-17 beta CA , the formation of labeled DHT was inhibited by more than 80 % .
	manualset3
203374	9	417550	7	NULL	NULL	0	NULL	80 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When homogenates of hypothalami or anterior pituitary glands were incubated with ( 3H ) Testosterone in the presence of a 50-fold excess of testosterone-17 beta CA , the formation of labeled DHT was inhibited by more than 80 % .
	manualset3
203384	1	417551	7	NULL	NULL	0	NULL	human HepG2 hepatoma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	When human HepG2 hepatoma cells were pulsed with 125I-labeled high density lipoproteins ( HDL ) and chased in fresh medium , up to 65 % of the radioactivity released was precipitable with trichloroacetic acid .
	manualset3
203387	2	417551	7	NULL	NULL	0	NULL	125I-labeled high density lipoproteins ( HDL )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When human HepG2 hepatoma cells were pulsed with 125I-labeled high density lipoproteins ( HDL ) and chased in fresh medium , up to 65 % of the radioactivity released was precipitable with trichloroacetic acid .
	manualset3
203388	3	417551	7	NULL	NULL	0	NULL	fresh medium	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	When human HepG2 hepatoma cells were pulsed with 125I-labeled high density lipoproteins ( HDL ) and chased in fresh medium , up to 65 % of the radioactivity released was precipitable with trichloroacetic acid .
	manualset3
203391	4	417551	7	NULL	NULL	0	NULL	65 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When human HepG2 hepatoma cells were pulsed with 125I-labeled high density lipoproteins ( HDL ) and chased in fresh medium , up to 65 % of the radioactivity released was precipitable with trichloroacetic acid .
	manualset3
203392	5	417551	7	NULL	NULL	0	NULL	radioactivity	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When human HepG2 hepatoma cells were pulsed with 125I-labeled high density lipoproteins ( HDL ) and chased in fresh medium , up to 65 % of the radioactivity released was precipitable with trichloroacetic acid .
	manualset3
203393	6	417551	7	NULL	NULL	0	NULL	trichloroacetic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When human HepG2 hepatoma cells were pulsed with 125I-labeled high density lipoproteins ( HDL ) and chased in fresh medium , up to 65 % of the radioactivity released was precipitable with trichloroacetic acid .
	manualset3
203398	1	417552	7	NULL	NULL	0	NULL	TP capsules 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	When implanted with TP capsules and tested while sexually naive , all groups of female rats preferred females to males without differing statistically .
	manualset3
203399	2	417552	7	NULL	NULL	0	NULL	groups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When implanted with TP capsules and tested while sexually naive , all groups of female rats preferred females to males without differing statistically .
	manualset3
203401	3	417552	7	NULL	NULL	0	NULL	female rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When implanted with TP capsules and tested while sexually naive , all groups of female rats preferred females to males without differing statistically .
	manualset3
203403	4	417552	7	NULL	NULL	0	NULL	females	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When implanted with TP capsules and tested while sexually naive , all groups of female rats preferred females to males without differing statistically .
	manualset3
203404	5	417552	7	NULL	NULL	0	NULL	males	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When implanted with TP capsules and tested while sexually naive , all groups of female rats preferred females to males without differing statistically .
	manualset3
203405	1	417553	7	NULL	NULL	0	NULL	preceding cycle	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When in a preceding cycle a significant hematologic toxicity was observed , this patient was treated in the subsequent cycle with the same dose of chemotherapy in combination with GM-CSF 250 micrograms/m2/day from day 2-12 as a continuous infusion .
	manualset3
203406	2	417553	7	NULL	NULL	0	NULL	hematologic toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When in a preceding cycle a significant hematologic toxicity was observed , this patient was treated in the subsequent cycle with the same dose of chemotherapy in combination with GM-CSF 250 micrograms/m2/day from day 2-12 as a continuous infusion .
	manualset3
203407	3	417553	7	NULL	NULL	0	NULL	patient	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When in a preceding cycle a significant hematologic toxicity was observed , this patient was treated in the subsequent cycle with the same dose of chemotherapy in combination with GM-CSF 250 micrograms/m2/day from day 2-12 as a continuous infusion .
	manualset3
203408	4	417553	7	NULL	NULL	0	NULL	 subsequent cycle	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When in a preceding cycle a significant hematologic toxicity was observed , this patient was treated in the subsequent cycle with the same dose of chemotherapy in combination with GM-CSF 250 micrograms/m2/day from day 2-12 as a continuous infusion .
	manualset3
203409	5	417553	7	NULL	NULL	0	NULL	dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When in a preceding cycle a significant hematologic toxicity was observed , this patient was treated in the subsequent cycle with the same dose of chemotherapy in combination with GM-CSF 250 micrograms/m2/day from day 2-12 as a continuous infusion .
	manualset3
203410	6	417553	7	NULL	NULL	0	NULL	 chemotherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	When in a preceding cycle a significant hematologic toxicity was observed , this patient was treated in the subsequent cycle with the same dose of chemotherapy in combination with GM-CSF 250 micrograms/m2/day from day 2-12 as a continuous infusion .
	manualset3
203411	7	417553	7	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When in a preceding cycle a significant hematologic toxicity was observed , this patient was treated in the subsequent cycle with the same dose of chemotherapy in combination with GM-CSF 250 micrograms/m2/day from day 2-12 as a continuous infusion .
	manualset3
203412	8	417553	7	NULL	NULL	0	NULL	GM-CSF 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When in a preceding cycle a significant hematologic toxicity was observed , this patient was treated in the subsequent cycle with the same dose of chemotherapy in combination with GM-CSF 250 micrograms/m2/day from day 2-12 as a continuous infusion .
	manualset3
203413	9	417553	7	NULL	NULL	0	NULL	250 micrograms/m2/day	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	When in a preceding cycle a significant hematologic toxicity was observed , this patient was treated in the subsequent cycle with the same dose of chemotherapy in combination with GM-CSF 250 micrograms/m2/day from day 2-12 as a continuous infusion .
	manualset3
203414	10	417553	7	NULL	NULL	0	NULL	day 2-12	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	When in a preceding cycle a significant hematologic toxicity was observed , this patient was treated in the subsequent cycle with the same dose of chemotherapy in combination with GM-CSF 250 micrograms/m2/day from day 2-12 as a continuous infusion .
	manualset3
203415	11	417553	7	NULL	NULL	0	NULL	continuous infusion 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	When in a preceding cycle a significant hematologic toxicity was observed , this patient was treated in the subsequent cycle with the same dose of chemotherapy in combination with GM-CSF 250 micrograms/m2/day from day 2-12 as a continuous infusion .
	manualset3
203416	1	417554	7	NULL	NULL	0	NULL	 influenza	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When influenza was occurring in the community ( 1979 to 1980 and 1980 to 1981 ) , however , the risk of death from pneumonia in the unvaccinated group was three-fold higher than in the vaccinated group ( 60 % vs 18 % and 73 % vs 25 % , respectively ) .
	manualset3
203417	2	417554	7	NULL	NULL	0	NULL	community	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When influenza was occurring in the community ( 1979 to 1980 and 1980 to 1981 ) , however , the risk of death from pneumonia in the unvaccinated group was three-fold higher than in the vaccinated group ( 60 % vs 18 % and 73 % vs 25 % , respectively ) .
	manualset3
203418	3	417554	7	NULL	NULL	0	NULL	1979 to 1980	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	When influenza was occurring in the community ( 1979 to 1980 and 1980 to 1981 ) , however , the risk of death from pneumonia in the unvaccinated group was three-fold higher than in the vaccinated group ( 60 % vs 18 % and 73 % vs 25 % , respectively ) .
	manualset3
203419	4	417554	7	NULL	NULL	0	NULL	1980 to 1981	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	When influenza was occurring in the community ( 1979 to 1980 and 1980 to 1981 ) , however , the risk of death from pneumonia in the unvaccinated group was three-fold higher than in the vaccinated group ( 60 % vs 18 % and 73 % vs 25 % , respectively ) .
	manualset3
203420	5	417554	7	NULL	NULL	0	NULL	 risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When influenza was occurring in the community ( 1979 to 1980 and 1980 to 1981 ) , however , the risk of death from pneumonia in the unvaccinated group was three-fold higher than in the vaccinated group ( 60 % vs 18 % and 73 % vs 25 % , respectively ) .
	manualset3
203421	6	417554	7	NULL	NULL	0	NULL	 death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When influenza was occurring in the community ( 1979 to 1980 and 1980 to 1981 ) , however , the risk of death from pneumonia in the unvaccinated group was three-fold higher than in the vaccinated group ( 60 % vs 18 % and 73 % vs 25 % , respectively ) .
	manualset3
203422	7	417554	7	NULL	NULL	0	NULL	pneumonia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	When influenza was occurring in the community ( 1979 to 1980 and 1980 to 1981 ) , however , the risk of death from pneumonia in the unvaccinated group was three-fold higher than in the vaccinated group ( 60 % vs 18 % and 73 % vs 25 % , respectively ) .
	manualset3
203423	8	417554	7	NULL	NULL	0	NULL	unvaccinated group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When influenza was occurring in the community ( 1979 to 1980 and 1980 to 1981 ) , however , the risk of death from pneumonia in the unvaccinated group was three-fold higher than in the vaccinated group ( 60 % vs 18 % and 73 % vs 25 % , respectively ) .
	manualset3
203424	9	417554	7	NULL	NULL	0	NULL	three-fold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When influenza was occurring in the community ( 1979 to 1980 and 1980 to 1981 ) , however , the risk of death from pneumonia in the unvaccinated group was three-fold higher than in the vaccinated group ( 60 % vs 18 % and 73 % vs 25 % , respectively ) .
	manualset3
203425	10	417554	7	NULL	NULL	0	NULL	vaccinated group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When influenza was occurring in the community ( 1979 to 1980 and 1980 to 1981 ) , however , the risk of death from pneumonia in the unvaccinated group was three-fold higher than in the vaccinated group ( 60 % vs 18 % and 73 % vs 25 % , respectively ) .
	manualset3
203426	11	417554	7	NULL	NULL	0	NULL	60 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When influenza was occurring in the community ( 1979 to 1980 and 1980 to 1981 ) , however , the risk of death from pneumonia in the unvaccinated group was three-fold higher than in the vaccinated group ( 60 % vs 18 % and 73 % vs 25 % , respectively ) .
	manualset3
203427	12	417554	7	NULL	NULL	0	NULL	18 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When influenza was occurring in the community ( 1979 to 1980 and 1980 to 1981 ) , however , the risk of death from pneumonia in the unvaccinated group was three-fold higher than in the vaccinated group ( 60 % vs 18 % and 73 % vs 25 % , respectively ) .
	manualset3
203428	13	417554	7	NULL	NULL	0	NULL	73 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When influenza was occurring in the community ( 1979 to 1980 and 1980 to 1981 ) , however , the risk of death from pneumonia in the unvaccinated group was three-fold higher than in the vaccinated group ( 60 % vs 18 % and 73 % vs 25 % , respectively ) .
	manualset3
203429	14	417554	7	NULL	NULL	0	NULL	25 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When influenza was occurring in the community ( 1979 to 1980 and 1980 to 1981 ) , however , the risk of death from pneumonia in the unvaccinated group was three-fold higher than in the vaccinated group ( 60 % vs 18 % and 73 % vs 25 % , respectively ) .
	manualset3
203430	1	417555	7	NULL	NULL	0	NULL	 injections 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	When injections were restricted to the neostriatum , retrograde labeling was found in layer V of both SI cortices .
	manualset3
203431	2	417555	7	NULL	NULL	0	NULL	neostriatum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When injections were restricted to the neostriatum , retrograde labeling was found in layer V of both SI cortices .
	manualset3
203432	3	417555	7	NULL	NULL	0	NULL	 retrograde labeling 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When injections were restricted to the neostriatum , retrograde labeling was found in layer V of both SI cortices .
	manualset3
203433	4	417555	7	NULL	NULL	0	NULL	layer V	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When injections were restricted to the neostriatum , retrograde labeling was found in layer V of both SI cortices .
	manualset3
203434	5	417555	7	NULL	NULL	0	NULL	SI cortices	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When injections were restricted to the neostriatum , retrograde labeling was found in layer V of both SI cortices .
	manualset3
203435	1	417556	7	NULL	NULL	0	NULL	opine-positive root clones	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	All opine-positive root clones showed NPT II ( neomycin phosphotransferase ) activity .
	manualset3
203436	2	417556	7	NULL	NULL	0	NULL	NPT II ( neomycin phosphotransferase ) activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All opine-positive root clones showed NPT II ( neomycin phosphotransferase ) activity .
	manualset3
203437	1	417557	7	NULL	NULL	0	NULL	full-length Pitx2c	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When introduced into full-length Pitx2c , the mutation results in an only 25 % loss of transactivation activity .
	manualset3
203438	2	417557	7	NULL	NULL	0	NULL	mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When introduced into full-length Pitx2c , the mutation results in an only 25 % loss of transactivation activity .
	manualset3
203439	3	417557	7	NULL	NULL	0	NULL	 25 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When introduced into full-length Pitx2c , the mutation results in an only 25 % loss of transactivation activity .
	manualset3
203440	4	417557	7	NULL	NULL	0	NULL	loss	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When introduced into full-length Pitx2c , the mutation results in an only 25 % loss of transactivation activity .
	manualset3
203441	5	417557	7	NULL	NULL	0	NULL	transactivation activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When introduced into full-length Pitx2c , the mutation results in an only 25 % loss of transactivation activity .
	manualset3
203442	1	417558	7	NULL	NULL	0	NULL	 isoprenaline	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	When isoprenaline was applied for 100 min , a transient increase in ( Mg2 + ) i was observed during the initial 25 min , whilst concentrations of ATP ( ( ATP ) ) and phosphocreatine ( ( PCr ) ) decreased and ( Pi ) correspondingly increased .
	manualset3
203443	2	417558	7	NULL	NULL	0	NULL	100 min 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	When isoprenaline was applied for 100 min , a transient increase in ( Mg2 + ) i was observed during the initial 25 min , whilst concentrations of ATP ( ( ATP ) ) and phosphocreatine ( ( PCr ) ) decreased and ( Pi ) correspondingly increased .
	manualset3
203444	3	417558	7	NULL	NULL	0	NULL	transient increase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When isoprenaline was applied for 100 min , a transient increase in ( Mg2 + ) i was observed during the initial 25 min , whilst concentrations of ATP ( ( ATP ) ) and phosphocreatine ( ( PCr ) ) decreased and ( Pi ) correspondingly increased .
	manualset3
203445	4	417558	7	NULL	NULL	0	NULL	Mg2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	When isoprenaline was applied for 100 min , a transient increase in ( Mg2 + ) i was observed during the initial 25 min , whilst concentrations of ATP ( ( ATP ) ) and phosphocreatine ( ( PCr ) ) decreased and ( Pi ) correspondingly increased .
	manualset3
203446	5	417558	7	NULL	NULL	0	NULL	25 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	When isoprenaline was applied for 100 min , a transient increase in ( Mg2 + ) i was observed during the initial 25 min , whilst concentrations of ATP ( ( ATP ) ) and phosphocreatine ( ( PCr ) ) decreased and ( Pi ) correspondingly increased .
	manualset3
203447	6	417558	7	NULL	NULL	0	NULL	 concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When isoprenaline was applied for 100 min , a transient increase in ( Mg2 + ) i was observed during the initial 25 min , whilst concentrations of ATP ( ( ATP ) ) and phosphocreatine ( ( PCr ) ) decreased and ( Pi ) correspondingly increased .
	manualset3
203448	7	417558	7	NULL	NULL	0	NULL	 ATP ( ( ATP ) )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When isoprenaline was applied for 100 min , a transient increase in ( Mg2 + ) i was observed during the initial 25 min , whilst concentrations of ATP ( ( ATP ) ) and phosphocreatine ( ( PCr ) ) decreased and ( Pi ) correspondingly increased .
	manualset3
203449	8	417558	7	NULL	NULL	0	NULL	phosphocreatine ( ( PCr ) ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When isoprenaline was applied for 100 min , a transient increase in ( Mg2 + ) i was observed during the initial 25 min , whilst concentrations of ATP ( ( ATP ) ) and phosphocreatine ( ( PCr ) ) decreased and ( Pi ) correspondingly increased .
	manualset3
203450	9	417558	7	NULL	NULL	0	NULL	 Pi	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When isoprenaline was applied for 100 min , a transient increase in ( Mg2 + ) i was observed during the initial 25 min , whilst concentrations of ATP ( ( ATP ) ) and phosphocreatine ( ( PCr ) ) decreased and ( Pi ) correspondingly increased .
	manualset3
203451	1	417559	7	NULL	NULL	0	NULL	cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	When many cultures of Treponema pallidum , whether obtained from the testicular lesions produced in rabbits or directly from human cases of syphilis , are compared , certain definite differences in morphological character become apparent .
	manualset3
203452	2	417559	7	NULL	NULL	0	NULL	Treponema pallidum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When many cultures of Treponema pallidum , whether obtained from the testicular lesions produced in rabbits or directly from human cases of syphilis , are compared , certain definite differences in morphological character become apparent .
	manualset3
203453	3	417559	7	NULL	NULL	0	NULL	testicular lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When many cultures of Treponema pallidum , whether obtained from the testicular lesions produced in rabbits or directly from human cases of syphilis , are compared , certain definite differences in morphological character become apparent .
	manualset3
203454	4	417559	7	NULL	NULL	0	NULL	rabbits	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When many cultures of Treponema pallidum , whether obtained from the testicular lesions produced in rabbits or directly from human cases of syphilis , are compared , certain definite differences in morphological character become apparent .
	manualset3
203455	5	417559	7	NULL	NULL	0	NULL	 human cases	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When many cultures of Treponema pallidum , whether obtained from the testicular lesions produced in rabbits or directly from human cases of syphilis , are compared , certain definite differences in morphological character become apparent .
	manualset3
203456	6	417559	7	NULL	NULL	0	NULL	syphilis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When many cultures of Treponema pallidum , whether obtained from the testicular lesions produced in rabbits or directly from human cases of syphilis , are compared , certain definite differences in morphological character become apparent .
	manualset3
203457	7	417559	7	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	When many cultures of Treponema pallidum , whether obtained from the testicular lesions produced in rabbits or directly from human cases of syphilis , are compared , certain definite differences in morphological character become apparent .
	manualset3
203458	8	417559	7	NULL	NULL	0	NULL	morphological character	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When many cultures of Treponema pallidum , whether obtained from the testicular lesions produced in rabbits or directly from human cases of syphilis , are compared , certain definite differences in morphological character become apparent .
	manualset3
203459	1	417560	7	NULL	NULL	NULL	NULL	 morphine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When morphine combined with desipramine was decreased to a subthreshold dose , we observed pronounced antinociception when a subthreshold dose of serotonin was added .
	manualset3
203460	2	417560	7	NULL	NULL	NULL	NULL	desipramine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When morphine combined with desipramine was decreased to a subthreshold dose , we observed pronounced antinociception when a subthreshold dose of serotonin was added .
	manualset3
203461	3	417560	7	NULL	NULL	0	NULL	subthreshold dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When morphine combined with desipramine was decreased to a subthreshold dose , we observed pronounced antinociception when a subthreshold dose of serotonin was added .
	manualset3
203462	4	417560	7	NULL	NULL	0	NULL	antinociception	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When morphine combined with desipramine was decreased to a subthreshold dose , we observed pronounced antinociception when a subthreshold dose of serotonin was added .
	manualset3
203463	5	417560	7	NULL	NULL	0	NULL	subthreshold dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When morphine combined with desipramine was decreased to a subthreshold dose , we observed pronounced antinociception when a subthreshold dose of serotonin was added .
	manualset3
203464	6	417560	7	NULL	NULL	0	NULL	serotonin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	When morphine combined with desipramine was decreased to a subthreshold dose , we observed pronounced antinociception when a subthreshold dose of serotonin was added .
	manualset3
203465	1	417561	7	NULL	NULL	0	NULL	mouse monoclonal antibodies ( MAbs )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When mouse monoclonal antibodies ( MAbs ) are injected into patients they usually induce an immune response .
	manualset3
203466	2	417561	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When mouse monoclonal antibodies ( MAbs ) are injected into patients they usually induce an immune response .
	manualset3
203467	3	417561	7	NULL	NULL	0	NULL	 immune response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When mouse monoclonal antibodies ( MAbs ) are injected into patients they usually induce an immune response .
	manualset3
203468	1	417562	7	NULL	NULL	0	NULL	mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When mutations resulting in requirements for histidine , leucine , serine , and trytophan were introduced singly into the glycine mutant , transformants for the leucine , serine , and histidine markers could be obtained at will , but transformants for the tryptophan marker were not detected even though all four of the double mutants could be transformed to glycine independence .
	manualset3
203469	2	417562	7	NULL	NULL	0	NULL	 requirements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When mutations resulting in requirements for histidine , leucine , serine , and trytophan were introduced singly into the glycine mutant , transformants for the leucine , serine , and histidine markers could be obtained at will , but transformants for the tryptophan marker were not detected even though all four of the double mutants could be transformed to glycine independence .
	manualset3
203470	3	417562	7	NULL	NULL	0	NULL	histidine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	When mutations resulting in requirements for histidine , leucine , serine , and trytophan were introduced singly into the glycine mutant , transformants for the leucine , serine , and histidine markers could be obtained at will , but transformants for the tryptophan marker were not detected even though all four of the double mutants could be transformed to glycine independence .
	manualset3
203471	4	417562	7	NULL	NULL	0	NULL	leucine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	When mutations resulting in requirements for histidine , leucine , serine , and trytophan were introduced singly into the glycine mutant , transformants for the leucine , serine , and histidine markers could be obtained at will , but transformants for the tryptophan marker were not detected even though all four of the double mutants could be transformed to glycine independence .
	manualset3
203472	5	417562	7	NULL	NULL	0	NULL	serine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	When mutations resulting in requirements for histidine , leucine , serine , and trytophan were introduced singly into the glycine mutant , transformants for the leucine , serine , and histidine markers could be obtained at will , but transformants for the tryptophan marker were not detected even though all four of the double mutants could be transformed to glycine independence .
	manualset3
203473	6	417562	7	NULL	NULL	0	NULL	trytophan	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	When mutations resulting in requirements for histidine , leucine , serine , and trytophan were introduced singly into the glycine mutant , transformants for the leucine , serine , and histidine markers could be obtained at will , but transformants for the tryptophan marker were not detected even though all four of the double mutants could be transformed to glycine independence .
	manualset3
203474	7	417562	7	NULL	NULL	0	NULL	glycine mutant	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	When mutations resulting in requirements for histidine , leucine , serine , and trytophan were introduced singly into the glycine mutant , transformants for the leucine , serine , and histidine markers could be obtained at will , but transformants for the tryptophan marker were not detected even though all four of the double mutants could be transformed to glycine independence .
	manualset3
203475	8	417562	7	NULL	NULL	NULL	NULL	transformants	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When mutations resulting in requirements for histidine , leucine , serine , and trytophan were introduced singly into the glycine mutant , transformants for the leucine , serine , and histidine markers could be obtained at will , but transformants for the tryptophan marker were not detected even though all four of the double mutants could be transformed to glycine independence .
	manualset3
203476	9	417562	7	NULL	NULL	0	NULL	 leucine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	When mutations resulting in requirements for histidine , leucine , serine , and trytophan were introduced singly into the glycine mutant , transformants for the leucine , serine , and histidine markers could be obtained at will , but transformants for the tryptophan marker were not detected even though all four of the double mutants could be transformed to glycine independence .
	manualset3
203477	10	417562	7	NULL	NULL	0	NULL	serine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	When mutations resulting in requirements for histidine , leucine , serine , and trytophan were introduced singly into the glycine mutant , transformants for the leucine , serine , and histidine markers could be obtained at will , but transformants for the tryptophan marker were not detected even though all four of the double mutants could be transformed to glycine independence .
	manualset3
203478	11	417562	7	NULL	NULL	NULL	NULL	histidine marker	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When mutations resulting in requirements for histidine , leucine , serine , and trytophan were introduced singly into the glycine mutant , transformants for the leucine , serine , and histidine markers could be obtained at will , but transformants for the tryptophan marker were not detected even though all four of the double mutants could be transformed to glycine independence .
	manualset3
203479	12	417562	7	NULL	NULL	0	NULL	transformants	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	When mutations resulting in requirements for histidine , leucine , serine , and trytophan were introduced singly into the glycine mutant , transformants for the leucine , serine , and histidine markers could be obtained at will , but transformants for the tryptophan marker were not detected even though all four of the double mutants could be transformed to glycine independence .
	manualset3
203480	13	417562	7	NULL	NULL	0	NULL	tryptophan marker	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	When mutations resulting in requirements for histidine , leucine , serine , and trytophan were introduced singly into the glycine mutant , transformants for the leucine , serine , and histidine markers could be obtained at will , but transformants for the tryptophan marker were not detected even though all four of the double mutants could be transformed to glycine independence .
	manualset3
203481	14	417562	7	NULL	NULL	0	NULL	four	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When mutations resulting in requirements for histidine , leucine , serine , and trytophan were introduced singly into the glycine mutant , transformants for the leucine , serine , and histidine markers could be obtained at will , but transformants for the tryptophan marker were not detected even though all four of the double mutants could be transformed to glycine independence .
	manualset3
203482	15	417562	7	NULL	NULL	0	NULL	double mutants	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	When mutations resulting in requirements for histidine , leucine , serine , and trytophan were introduced singly into the glycine mutant , transformants for the leucine , serine , and histidine markers could be obtained at will , but transformants for the tryptophan marker were not detected even though all four of the double mutants could be transformed to glycine independence .
	manualset3
203483	16	417562	7	NULL	NULL	0	NULL	glycine independence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When mutations resulting in requirements for histidine , leucine , serine , and trytophan were introduced singly into the glycine mutant , transformants for the leucine , serine , and histidine markers could be obtained at will , but transformants for the tryptophan marker were not detected even though all four of the double mutants could be transformed to glycine independence .
	manualset3
203484	1	417563	7	NULL	NULL	0	NULL	novobiocin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	When novobiocin is added after induction , transcription appears to be rapidly turned off , and the chromatin organization of the 87A7 locus is `` fixed '' in an `` active '' configuration .
	manualset3
203485	2	417563	7	NULL	NULL	NULL	NULL	induction 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When novobiocin is added after induction , transcription appears to be rapidly turned off , and the chromatin organization of the 87A7 locus is `` fixed '' in an `` active '' configuration .
	manualset3
203486	3	417563	7	NULL	NULL	0	NULL	transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When novobiocin is added after induction , transcription appears to be rapidly turned off , and the chromatin organization of the 87A7 locus is `` fixed '' in an `` active '' configuration .
	manualset3
203487	4	417563	7	NULL	NULL	0	NULL	chromatin organization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When novobiocin is added after induction , transcription appears to be rapidly turned off , and the chromatin organization of the 87A7 locus is `` fixed '' in an `` active '' configuration .
	manualset3
203488	5	417563	7	NULL	NULL	0	NULL	87A7 locus 	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	When novobiocin is added after induction , transcription appears to be rapidly turned off , and the chromatin organization of the 87A7 locus is `` fixed '' in an `` active '' configuration .
	manualset3
203489	6	417563	7	NULL	NULL	0	NULL	`` active '' configuration	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When novobiocin is added after induction , transcription appears to be rapidly turned off , and the chromatin organization of the 87A7 locus is `` fixed '' in an `` active '' configuration .
	manualset3
203490	1	417564	7	NULL	NULL	0	NULL	 nuclei 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	When nuclei were incubated at 29 degrees C for 1 h , about 27 per cent of the newly synthesized RNA was released into the medium outside the nucleus .
	manualset3
203491	2	417564	7	NULL	NULL	0	NULL	29 degrees C	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When nuclei were incubated at 29 degrees C for 1 h , about 27 per cent of the newly synthesized RNA was released into the medium outside the nucleus .
	manualset3
203492	3	417564	7	NULL	NULL	0	NULL	1 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	When nuclei were incubated at 29 degrees C for 1 h , about 27 per cent of the newly synthesized RNA was released into the medium outside the nucleus .
	manualset3
203493	4	417564	7	NULL	NULL	0	NULL	 27 per cent	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When nuclei were incubated at 29 degrees C for 1 h , about 27 per cent of the newly synthesized RNA was released into the medium outside the nucleus .
	manualset3
203494	5	417564	7	NULL	NULL	0	NULL	newly synthesized RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	When nuclei were incubated at 29 degrees C for 1 h , about 27 per cent of the newly synthesized RNA was released into the medium outside the nucleus .
	manualset3
203495	6	417564	7	NULL	NULL	0	NULL	medium	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	When nuclei were incubated at 29 degrees C for 1 h , about 27 per cent of the newly synthesized RNA was released into the medium outside the nucleus .
	manualset3
203496	7	417564	7	NULL	NULL	0	NULL	nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	When nuclei were incubated at 29 degrees C for 1 h , about 27 per cent of the newly synthesized RNA was released into the medium outside the nucleus .
	manualset3
203497	1	417565	7	NULL	NULL	0	NULL	organisms 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	All organisms have mass , transform , store and use biochemical energy and obey the most fundamental of all laws -- the laws of thermodynamics .
	manualset3
203498	2	417565	7	NULL	NULL	0	NULL	mass	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All organisms have mass , transform , store and use biochemical energy and obey the most fundamental of all laws -- the laws of thermodynamics .
	manualset3
203499	3	417565	7	NULL	NULL	NULL	NULL	biochemical energy 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	All organisms have mass , transform , store and use biochemical energy and obey the most fundamental of all laws -- the laws of thermodynamics .
	manualset3
203500	4	417565	7	NULL	NULL	NULL	NULL	 all laws	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	All organisms have mass , transform , store and use biochemical energy and obey the most fundamental of all laws -- the laws of thermodynamics .
	manualset3
203502	6	417565	7	NULL	NULL	NULL	NULL	laws of thermodynamics	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	All organisms have mass , transform , store and use biochemical energy and obey the most fundamental of all laws -- the laws of thermodynamics .
	manualset3
203503	1	417566	7	NULL	NULL	0	NULL	Cav-1-negative PCa cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	When overexpressed in Cav-1-negative PCa cells , Cav-1 ( C133/143/156S ) caused a reduction of both Src and Akt levels , as well as of their active , phosphorylated forms , in comparison with wild type Cav-1 .
	manualset3
203504	2	417566	7	NULL	NULL	0	NULL	Cav-1 ( C133/143/156S )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When overexpressed in Cav-1-negative PCa cells , Cav-1 ( C133/143/156S ) caused a reduction of both Src and Akt levels , as well as of their active , phosphorylated forms , in comparison with wild type Cav-1 .
	manualset3
203505	3	417566	7	NULL	NULL	0	NULL	 Src levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When overexpressed in Cav-1-negative PCa cells , Cav-1 ( C133/143/156S ) caused a reduction of both Src and Akt levels , as well as of their active , phosphorylated forms , in comparison with wild type Cav-1 .
	manualset3
203506	4	417566	7	NULL	NULL	0	NULL	Akt levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When overexpressed in Cav-1-negative PCa cells , Cav-1 ( C133/143/156S ) caused a reduction of both Src and Akt levels , as well as of their active , phosphorylated forms , in comparison with wild type Cav-1 .
	manualset3
203507	5	417566	7	NULL	NULL	0	NULL	 phosphorylated forms 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When overexpressed in Cav-1-negative PCa cells , Cav-1 ( C133/143/156S ) caused a reduction of both Src and Akt levels , as well as of their active , phosphorylated forms , in comparison with wild type Cav-1 .
	manualset3
203508	6	417566	7	NULL	NULL	0	NULL	comparison 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	When overexpressed in Cav-1-negative PCa cells , Cav-1 ( C133/143/156S ) caused a reduction of both Src and Akt levels , as well as of their active , phosphorylated forms , in comparison with wild type Cav-1 .
	manualset3
203509	7	417566	7	NULL	NULL	0	NULL	wild type Cav-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When overexpressed in Cav-1-negative PCa cells , Cav-1 ( C133/143/156S ) caused a reduction of both Src and Akt levels , as well as of their active , phosphorylated forms , in comparison with wild type Cav-1 .
	manualset3
203510	8	417566	7	NULL	NULL	0	NULL	reduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When overexpressed in Cav-1-negative PCa cells , Cav-1 ( C133/143/156S ) caused a reduction of both Src and Akt levels , as well as of their active , phosphorylated forms , in comparison with wild type Cav-1 .
	manualset3
203511	1	417567	7	NULL	NULL	0	NULL	 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	When place cells are recorded from rats running on an elevated T-maze inside a curtained enclosure that contains distinct , experimenter selected stimuli , rotations of the maze plus stimuli cause equal rotations of firing fields .
	manualset3
203512	2	417567	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When place cells are recorded from rats running on an elevated T-maze inside a curtained enclosure that contains distinct , experimenter selected stimuli , rotations of the maze plus stimuli cause equal rotations of firing fields .
	manualset3
203513	3	417567	7	NULL	NULL	0	NULL	elevated T-maze 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	When place cells are recorded from rats running on an elevated T-maze inside a curtained enclosure that contains distinct , experimenter selected stimuli , rotations of the maze plus stimuli cause equal rotations of firing fields .
	manualset3
203514	4	417567	7	NULL	NULL	0	NULL	curtained enclosure	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	When place cells are recorded from rats running on an elevated T-maze inside a curtained enclosure that contains distinct , experimenter selected stimuli , rotations of the maze plus stimuli cause equal rotations of firing fields .
	manualset3
203515	5	417567	7	NULL	NULL	0	NULL	experimenter	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	When place cells are recorded from rats running on an elevated T-maze inside a curtained enclosure that contains distinct , experimenter selected stimuli , rotations of the maze plus stimuli cause equal rotations of firing fields .
	manualset3
203516	6	417567	7	NULL	NULL	0	NULL	stimuli	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	When place cells are recorded from rats running on an elevated T-maze inside a curtained enclosure that contains distinct , experimenter selected stimuli , rotations of the maze plus stimuli cause equal rotations of firing fields .
	manualset3
203517	7	417567	7	NULL	NULL	0	NULL	 rotations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When place cells are recorded from rats running on an elevated T-maze inside a curtained enclosure that contains distinct , experimenter selected stimuli , rotations of the maze plus stimuli cause equal rotations of firing fields .
	manualset3
203518	8	417567	7	NULL	NULL	0	NULL	maze	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	When place cells are recorded from rats running on an elevated T-maze inside a curtained enclosure that contains distinct , experimenter selected stimuli , rotations of the maze plus stimuli cause equal rotations of firing fields .
	manualset3
203519	9	417567	7	NULL	NULL	0	NULL	 stimuli 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	When place cells are recorded from rats running on an elevated T-maze inside a curtained enclosure that contains distinct , experimenter selected stimuli , rotations of the maze plus stimuli cause equal rotations of firing fields .
	manualset3
203520	10	417567	7	NULL	NULL	0	NULL	equal rotations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When place cells are recorded from rats running on an elevated T-maze inside a curtained enclosure that contains distinct , experimenter selected stimuli , rotations of the maze plus stimuli cause equal rotations of firing fields .
	manualset3
203521	11	417567	7	NULL	NULL	0	NULL	firing fields	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	When place cells are recorded from rats running on an elevated T-maze inside a curtained enclosure that contains distinct , experimenter selected stimuli , rotations of the maze plus stimuli cause equal rotations of firing fields .
	manualset3
203522	1	417568	7	NULL	NULL	0	NULL	risk factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When possible the risk factors has to be eliminated , arterial hypertension , diabetes mellitus and dyslipidemia have to be treated orderly .
	manualset3
203523	2	417568	7	NULL	NULL	0	NULL	arterial hypertension	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	When possible the risk factors has to be eliminated , arterial hypertension , diabetes mellitus and dyslipidemia have to be treated orderly .
	manualset3
203524	3	417568	7	NULL	NULL	0	NULL	diabetes mellitus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	When possible the risk factors has to be eliminated , arterial hypertension , diabetes mellitus and dyslipidemia have to be treated orderly .
	manualset3
203525	4	417568	7	NULL	NULL	0	NULL	dyslipidemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	When possible the risk factors has to be eliminated , arterial hypertension , diabetes mellitus and dyslipidemia have to be treated orderly .
	manualset3
203526	1	417569	7	NULL	NULL	0	NULL	protein adsorption sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	When potential protein adsorption sites on the substratum were covered with bovine serum albumin before initial human fibroblasts attachment , their subsequent attachment to the substratum was prevented .
	manualset3
203527	2	417569	7	NULL	NULL	NULL	NULL	substratum	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When potential protein adsorption sites on the substratum were covered with bovine serum albumin before initial human fibroblasts attachment , their subsequent attachment to the substratum was prevented .
	manualset3
203528	3	417569	7	NULL	NULL	0	NULL	bovine serum albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When potential protein adsorption sites on the substratum were covered with bovine serum albumin before initial human fibroblasts attachment , their subsequent attachment to the substratum was prevented .
	manualset3
203529	4	417569	7	NULL	NULL	0	NULL	human fibroblasts attachment	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When potential protein adsorption sites on the substratum were covered with bovine serum albumin before initial human fibroblasts attachment , their subsequent attachment to the substratum was prevented .
	manualset3
203530	5	417569	7	NULL	NULL	0	NULL	subsequent attachment	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When potential protein adsorption sites on the substratum were covered with bovine serum albumin before initial human fibroblasts attachment , their subsequent attachment to the substratum was prevented .
	manualset3
203531	6	417569	7	NULL	NULL	0	NULL	substratum	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When potential protein adsorption sites on the substratum were covered with bovine serum albumin before initial human fibroblasts attachment , their subsequent attachment to the substratum was prevented .
	manualset3
203532	1	417570	7	NULL	NULL	0	NULL	poultry litter	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When poultry litter is landspread , steroidal hormones present in the litter may reach surface waters , where they may have undesirable biological effects .
	manualset3
203533	2	417570	7	NULL	NULL	0	NULL	landspread	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When poultry litter is landspread , steroidal hormones present in the litter may reach surface waters , where they may have undesirable biological effects .
	manualset3
203534	3	417570	7	NULL	NULL	0	NULL	steroidal hormones	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When poultry litter is landspread , steroidal hormones present in the litter may reach surface waters , where they may have undesirable biological effects .
	manualset3
203535	4	417570	7	NULL	NULL	0	NULL	litter 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When poultry litter is landspread , steroidal hormones present in the litter may reach surface waters , where they may have undesirable biological effects .
	manualset3
203536	5	417570	7	NULL	NULL	0	NULL	surface waters	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When poultry litter is landspread , steroidal hormones present in the litter may reach surface waters , where they may have undesirable biological effects .
	manualset3
203537	6	417570	7	NULL	NULL	0	NULL	undesirable biological effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When poultry litter is landspread , steroidal hormones present in the litter may reach surface waters , where they may have undesirable biological effects .
	manualset3
203538	1	417571	7	NULL	NULL	0	NULL	sapling	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When sapling grew up as young tree , its adventitious root stretched into soil to assimilate the nutrient and water , and it became independence individual .
	manualset3
203539	2	417571	7	NULL	NULL	0	NULL	young tree	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When sapling grew up as young tree , its adventitious root stretched into soil to assimilate the nutrient and water , and it became independence individual .
	manualset3
203540	3	417571	7	NULL	NULL	0	NULL	adventitious root 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When sapling grew up as young tree , its adventitious root stretched into soil to assimilate the nutrient and water , and it became independence individual .
	manualset3
203541	4	417571	7	NULL	NULL	0	NULL	soil 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	When sapling grew up as young tree , its adventitious root stretched into soil to assimilate the nutrient and water , and it became independence individual .
	manualset3
203542	5	417571	7	NULL	NULL	0	NULL	nutrient 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When sapling grew up as young tree , its adventitious root stretched into soil to assimilate the nutrient and water , and it became independence individual .
	manualset3
203543	6	417571	7	NULL	NULL	0	NULL	 water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When sapling grew up as young tree , its adventitious root stretched into soil to assimilate the nutrient and water , and it became independence individual .
	manualset3
203544	7	417571	7	NULL	NULL	0	NULL	 individual	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	When sapling grew up as young tree , its adventitious root stretched into soil to assimilate the nutrient and water , and it became independence individual .
	manualset3
203545	1	417572	7	NULL	NULL	0	NULL	 K ( + )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	When some K ( + ) was present with high concentrations of Na ( + ) the inward currents were larger than with K ( + ) or Na ( + ) alone .
	manualset3
203546	2	417572	7	NULL	NULL	0	NULL	high concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When some K ( + ) was present with high concentrations of Na ( + ) the inward currents were larger than with K ( + ) or Na ( + ) alone .
	manualset3
203547	3	417572	7	NULL	NULL	0	NULL	Na ( + )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	When some K ( + ) was present with high concentrations of Na ( + ) the inward currents were larger than with K ( + ) or Na ( + ) alone .
	manualset3
203548	4	417572	7	NULL	NULL	0	NULL	inward currents	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When some K ( + ) was present with high concentrations of Na ( + ) the inward currents were larger than with K ( + ) or Na ( + ) alone .
	manualset3
203549	5	417572	7	NULL	NULL	0	NULL	K ( + )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	When some K ( + ) was present with high concentrations of Na ( + ) the inward currents were larger than with K ( + ) or Na ( + ) alone .
	manualset3
203550	6	417572	7	NULL	NULL	0	NULL	Na ( + ) 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	When some K ( + ) was present with high concentrations of Na ( + ) the inward currents were larger than with K ( + ) or Na ( + ) alone .
	manualset3
203551	1	417573	7	NULL	NULL	0	NULL	parameters	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	All parameters were unaltered because of poult sex .
	manualset3
203552	2	417573	7	NULL	NULL	NULL	NULL	poult sex	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	All parameters were unaltered because of poult sex .
	manualset3
203553	1	417574	7	NULL	NULL	0	NULL	spleen cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	When spleen cells from rats that had been treated with RP-3 at the time of immunization were used for local transfer of DTH , footpad swelling was significantly less than that induced by spleen cells from the RP-3-untreated immune rats .
	manualset3
203554	2	417574	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When spleen cells from rats that had been treated with RP-3 at the time of immunization were used for local transfer of DTH , footpad swelling was significantly less than that induced by spleen cells from the RP-3-untreated immune rats .
	manualset3
203555	3	417574	7	NULL	NULL	0	NULL	RP-3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When spleen cells from rats that had been treated with RP-3 at the time of immunization were used for local transfer of DTH , footpad swelling was significantly less than that induced by spleen cells from the RP-3-untreated immune rats .
	manualset3
203556	4	417574	7	NULL	NULL	0	NULL	 time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	When spleen cells from rats that had been treated with RP-3 at the time of immunization were used for local transfer of DTH , footpad swelling was significantly less than that induced by spleen cells from the RP-3-untreated immune rats .
	manualset3
203557	5	417574	7	NULL	NULL	0	NULL	 immunization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	When spleen cells from rats that had been treated with RP-3 at the time of immunization were used for local transfer of DTH , footpad swelling was significantly less than that induced by spleen cells from the RP-3-untreated immune rats .
	manualset3
203558	6	417574	7	NULL	NULL	NULL	NULL	 local transfer	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When spleen cells from rats that had been treated with RP-3 at the time of immunization were used for local transfer of DTH , footpad swelling was significantly less than that induced by spleen cells from the RP-3-untreated immune rats .
	manualset3
203559	7	417574	7	NULL	NULL	NULL	NULL	DTH	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When spleen cells from rats that had been treated with RP-3 at the time of immunization were used for local transfer of DTH , footpad swelling was significantly less than that induced by spleen cells from the RP-3-untreated immune rats .
	manualset3
203560	8	417574	7	NULL	NULL	0	NULL	footpad swelling	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When spleen cells from rats that had been treated with RP-3 at the time of immunization were used for local transfer of DTH , footpad swelling was significantly less than that induced by spleen cells from the RP-3-untreated immune rats .
	manualset3
203561	9	417574	7	NULL	NULL	0	NULL	spleen cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	When spleen cells from rats that had been treated with RP-3 at the time of immunization were used for local transfer of DTH , footpad swelling was significantly less than that induced by spleen cells from the RP-3-untreated immune rats .
	manualset3
203562	10	417574	7	NULL	NULL	0	NULL	RP-3-untreated immune rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When spleen cells from rats that had been treated with RP-3 at the time of immunization were used for local transfer of DTH , footpad swelling was significantly less than that induced by spleen cells from the RP-3-untreated immune rats .
	manualset3
203563	1	417575	7	NULL	NULL	0	NULL	angiogenic activities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When tested on other angiogenic activities mediated by VEGF , survivin antisense treatment induced rapid regression of three-dimensional vascular capillary networks , but did not affect EC migration/chemotaxis .
	manualset3
203564	2	417575	7	NULL	NULL	0	NULL	VEGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When tested on other angiogenic activities mediated by VEGF , survivin antisense treatment induced rapid regression of three-dimensional vascular capillary networks , but did not affect EC migration/chemotaxis .
	manualset3
203565	3	417575	7	NULL	NULL	0	NULL	survivin antisense treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	When tested on other angiogenic activities mediated by VEGF , survivin antisense treatment induced rapid regression of three-dimensional vascular capillary networks , but did not affect EC migration/chemotaxis .
	manualset3
203566	4	417575	7	NULL	NULL	0	NULL	 rapid regression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When tested on other angiogenic activities mediated by VEGF , survivin antisense treatment induced rapid regression of three-dimensional vascular capillary networks , but did not affect EC migration/chemotaxis .
	manualset3
203567	5	417575	7	NULL	NULL	0	NULL	three-dimensional vascular capillary networks	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When tested on other angiogenic activities mediated by VEGF , survivin antisense treatment induced rapid regression of three-dimensional vascular capillary networks , but did not affect EC migration/chemotaxis .
	manualset3
203568	6	417575	7	NULL	NULL	0	NULL	EC migration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When tested on other angiogenic activities mediated by VEGF , survivin antisense treatment induced rapid regression of three-dimensional vascular capillary networks , but did not affect EC migration/chemotaxis .
	manualset3
203569	7	417575	7	NULL	NULL	0	NULL	EC chemotaxis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When tested on other angiogenic activities mediated by VEGF , survivin antisense treatment induced rapid regression of three-dimensional vascular capillary networks , but did not affect EC migration/chemotaxis .
	manualset3
203570	1	417576	7	NULL	NULL	NULL	NULL	testing thermal vasomotor responses	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When testing thermal vasomotor responses by stepwise cooling of isolated carotid arteries , a temperature-proportional dilatation was observed while heating induced the opposite response : a marked vasoconstriction .
	manualset3
203571	2	417576	7	NULL	NULL	0	NULL	stepwise cooling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	When testing thermal vasomotor responses by stepwise cooling of isolated carotid arteries , a temperature-proportional dilatation was observed while heating induced the opposite response : a marked vasoconstriction .
	manualset3
203572	3	417576	7	NULL	NULL	0	NULL	isolated carotid arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When testing thermal vasomotor responses by stepwise cooling of isolated carotid arteries , a temperature-proportional dilatation was observed while heating induced the opposite response : a marked vasoconstriction .
	manualset3
203573	4	417576	7	NULL	NULL	0	NULL	 temperature-proportional dilatation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When testing thermal vasomotor responses by stepwise cooling of isolated carotid arteries , a temperature-proportional dilatation was observed while heating induced the opposite response : a marked vasoconstriction .
	manualset3
203574	5	417576	7	NULL	NULL	0	NULL	 heating	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When testing thermal vasomotor responses by stepwise cooling of isolated carotid arteries , a temperature-proportional dilatation was observed while heating induced the opposite response : a marked vasoconstriction .
	manualset3
203575	6	417576	7	NULL	NULL	0	NULL	opposite response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When testing thermal vasomotor responses by stepwise cooling of isolated carotid arteries , a temperature-proportional dilatation was observed while heating induced the opposite response : a marked vasoconstriction .
	manualset3
203576	7	417576	7	NULL	NULL	0	NULL	vasoconstriction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When testing thermal vasomotor responses by stepwise cooling of isolated carotid arteries , a temperature-proportional dilatation was observed while heating induced the opposite response : a marked vasoconstriction .
	manualset3
203577	1	417577	7	NULL	NULL	0	NULL	 2 drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	When the 2 drugs were combined , the beneficial effects of each drug on the trabecular microarchitecture were maintained , resulting in their additive effects on bone strength .
	manualset3
203578	2	417577	7	NULL	NULL	0	NULL	beneficial effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When the 2 drugs were combined , the beneficial effects of each drug on the trabecular microarchitecture were maintained , resulting in their additive effects on bone strength .
	manualset3
203579	3	417577	7	NULL	NULL	0	NULL	drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	When the 2 drugs were combined , the beneficial effects of each drug on the trabecular microarchitecture were maintained , resulting in their additive effects on bone strength .
	manualset3
203580	4	417577	7	NULL	NULL	0	NULL	 trabecular microarchitecture	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When the 2 drugs were combined , the beneficial effects of each drug on the trabecular microarchitecture were maintained , resulting in their additive effects on bone strength .
	manualset3
203581	5	417577	7	NULL	NULL	0	NULL	additive effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When the 2 drugs were combined , the beneficial effects of each drug on the trabecular microarchitecture were maintained , resulting in their additive effects on bone strength .
	manualset3
203582	6	417577	7	NULL	NULL	0	NULL	bone strength	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When the 2 drugs were combined , the beneficial effects of each drug on the trabecular microarchitecture were maintained , resulting in their additive effects on bone strength .
	manualset3
203583	1	417578	7	NULL	NULL	0	NULL	aluminium content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When the aluminium content of the water supply to our Haemodialysis Unit rose from less than 0.5 mumol/l to 6 mumol/l over a two month period , we carried out bone biopsies and desferrioxamine infusion tests on twelve ( 12 ) patients who had been on hemodialysis for less than one year ( mean 8 months ) and had normal serum aluminium levels .
	manualset3
203584	2	417578	7	NULL	NULL	0	NULL	water supply 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When the aluminium content of the water supply to our Haemodialysis Unit rose from less than 0.5 mumol/l to 6 mumol/l over a two month period , we carried out bone biopsies and desferrioxamine infusion tests on twelve ( 12 ) patients who had been on hemodialysis for less than one year ( mean 8 months ) and had normal serum aluminium levels .
	manualset3
203585	3	417578	7	NULL	NULL	0	NULL	Haemodialysis Unit	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	When the aluminium content of the water supply to our Haemodialysis Unit rose from less than 0.5 mumol/l to 6 mumol/l over a two month period , we carried out bone biopsies and desferrioxamine infusion tests on twelve ( 12 ) patients who had been on hemodialysis for less than one year ( mean 8 months ) and had normal serum aluminium levels .
	manualset3
203586	4	417578	7	NULL	NULL	0	NULL	 0.5 mumol/l	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	When the aluminium content of the water supply to our Haemodialysis Unit rose from less than 0.5 mumol/l to 6 mumol/l over a two month period , we carried out bone biopsies and desferrioxamine infusion tests on twelve ( 12 ) patients who had been on hemodialysis for less than one year ( mean 8 months ) and had normal serum aluminium levels .
	manualset3
203587	5	417578	7	NULL	NULL	0	NULL	6 mumol/l	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	When the aluminium content of the water supply to our Haemodialysis Unit rose from less than 0.5 mumol/l to 6 mumol/l over a two month period , we carried out bone biopsies and desferrioxamine infusion tests on twelve ( 12 ) patients who had been on hemodialysis for less than one year ( mean 8 months ) and had normal serum aluminium levels .
	manualset3
203588	6	417578	7	NULL	NULL	0	NULL	two month period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	When the aluminium content of the water supply to our Haemodialysis Unit rose from less than 0.5 mumol/l to 6 mumol/l over a two month period , we carried out bone biopsies and desferrioxamine infusion tests on twelve ( 12 ) patients who had been on hemodialysis for less than one year ( mean 8 months ) and had normal serum aluminium levels .
	manualset3
203589	7	417578	7	NULL	NULL	0	NULL	bone biopsies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	When the aluminium content of the water supply to our Haemodialysis Unit rose from less than 0.5 mumol/l to 6 mumol/l over a two month period , we carried out bone biopsies and desferrioxamine infusion tests on twelve ( 12 ) patients who had been on hemodialysis for less than one year ( mean 8 months ) and had normal serum aluminium levels .
	manualset3
203590	8	417578	7	NULL	NULL	0	NULL	desferrioxamine infusion tests	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	When the aluminium content of the water supply to our Haemodialysis Unit rose from less than 0.5 mumol/l to 6 mumol/l over a two month period , we carried out bone biopsies and desferrioxamine infusion tests on twelve ( 12 ) patients who had been on hemodialysis for less than one year ( mean 8 months ) and had normal serum aluminium levels .
	manualset3
203591	9	417578	7	NULL	NULL	0	NULL	twelve ( 12 ) patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When the aluminium content of the water supply to our Haemodialysis Unit rose from less than 0.5 mumol/l to 6 mumol/l over a two month period , we carried out bone biopsies and desferrioxamine infusion tests on twelve ( 12 ) patients who had been on hemodialysis for less than one year ( mean 8 months ) and had normal serum aluminium levels .
	manualset3
203592	10	417578	7	NULL	NULL	0	NULL	hemodialysis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	When the aluminium content of the water supply to our Haemodialysis Unit rose from less than 0.5 mumol/l to 6 mumol/l over a two month period , we carried out bone biopsies and desferrioxamine infusion tests on twelve ( 12 ) patients who had been on hemodialysis for less than one year ( mean 8 months ) and had normal serum aluminium levels .
	manualset3
203593	11	417578	7	NULL	NULL	0	NULL	one year	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	When the aluminium content of the water supply to our Haemodialysis Unit rose from less than 0.5 mumol/l to 6 mumol/l over a two month period , we carried out bone biopsies and desferrioxamine infusion tests on twelve ( 12 ) patients who had been on hemodialysis for less than one year ( mean 8 months ) and had normal serum aluminium levels .
	manualset3
203594	12	417578	7	NULL	NULL	0	NULL	8 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	When the aluminium content of the water supply to our Haemodialysis Unit rose from less than 0.5 mumol/l to 6 mumol/l over a two month period , we carried out bone biopsies and desferrioxamine infusion tests on twelve ( 12 ) patients who had been on hemodialysis for less than one year ( mean 8 months ) and had normal serum aluminium levels .
	manualset3
203595	13	417578	7	NULL	NULL	0	NULL	normal serum aluminium levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When the aluminium content of the water supply to our Haemodialysis Unit rose from less than 0.5 mumol/l to 6 mumol/l over a two month period , we carried out bone biopsies and desferrioxamine infusion tests on twelve ( 12 ) patients who had been on hemodialysis for less than one year ( mean 8 months ) and had normal serum aluminium levels .
	manualset3
203596	1	417579	7	NULL	NULL	0	NULL	segmentation time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	When the available segmentation time is fixed , both AMAS and ALMAS perform significantly better than MAS .
	manualset3
203597	2	417579	7	NULL	NULL	0	NULL	AMAS	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	When the available segmentation time is fixed , both AMAS and ALMAS perform significantly better than MAS .
	manualset3
203598	3	417579	7	NULL	NULL	0	NULL	ALMAS 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	When the available segmentation time is fixed , both AMAS and ALMAS perform significantly better than MAS .
	manualset3
203599	4	417579	7	NULL	NULL	0	NULL	MAS	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	When the available segmentation time is fixed , both AMAS and ALMAS perform significantly better than MAS .
	manualset3
203600	1	417580	7	NULL	NULL	NULL	NULL	coiled tube	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When the coiled tube is filled with one phase of a two-phase system and fed with the other phase , phase-interchange takes place in each turn of the coil , leaving a segment of the former phase as the stationary phase .
	manualset3
203601	2	417580	7	NULL	NULL	0	NULL	one phase of a two-phase system	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	When the coiled tube is filled with one phase of a two-phase system and fed with the other phase , phase-interchange takes place in each turn of the coil , leaving a segment of the former phase as the stationary phase .
	manualset3
203602	3	417580	7	NULL	NULL	0	NULL	phase-interchange	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When the coiled tube is filled with one phase of a two-phase system and fed with the other phase , phase-interchange takes place in each turn of the coil , leaving a segment of the former phase as the stationary phase .
	manualset3
203603	4	417580	7	NULL	NULL	NULL	NULL	turn of the coil	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When the coiled tube is filled with one phase of a two-phase system and fed with the other phase , phase-interchange takes place in each turn of the coil , leaving a segment of the former phase as the stationary phase .
	manualset3
203605	6	417580	7	NULL	NULL	0	NULL	 segment	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	When the coiled tube is filled with one phase of a two-phase system and fed with the other phase , phase-interchange takes place in each turn of the coil , leaving a segment of the former phase as the stationary phase .
	manualset3
203606	7	417580	7	NULL	NULL	0	NULL	former phase	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	When the coiled tube is filled with one phase of a two-phase system and fed with the other phase , phase-interchange takes place in each turn of the coil , leaving a segment of the former phase as the stationary phase .
	manualset3
203607	8	417580	7	NULL	NULL	0	NULL	 stationary phase	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	When the coiled tube is filled with one phase of a two-phase system and fed with the other phase , phase-interchange takes place in each turn of the coil , leaving a segment of the former phase as the stationary phase .
	manualset3
203608	1	417581	7	NULL	NULL	0	NULL	conditioning stimuli	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	When the conditioning and test stimuli were of equal frequencies , the test response was markedly suppressed at short interstimulus intervals ; complete recovery appeared at intervals from about 2 ms ( when two stimuli were of equal intensity ) to 10-20 ms ( when the conditioning stimulus exceeded the test by up to 40 dB ) .
	manualset3
203609	2	417581	7	NULL	NULL	0	NULL	test stimuli	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	When the conditioning and test stimuli were of equal frequencies , the test response was markedly suppressed at short interstimulus intervals ; complete recovery appeared at intervals from about 2 ms ( when two stimuli were of equal intensity ) to 10-20 ms ( when the conditioning stimulus exceeded the test by up to 40 dB ) .
	manualset3
203611	3	417581	7	NULL	NULL	0	NULL	equal frequencies	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When the conditioning and test stimuli were of equal frequencies , the test response was markedly suppressed at short interstimulus intervals ; complete recovery appeared at intervals from about 2 ms ( when two stimuli were of equal intensity ) to 10-20 ms ( when the conditioning stimulus exceeded the test by up to 40 dB ) .
	manualset3
203612	4	417581	7	NULL	NULL	0	NULL	test response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When the conditioning and test stimuli were of equal frequencies , the test response was markedly suppressed at short interstimulus intervals ; complete recovery appeared at intervals from about 2 ms ( when two stimuli were of equal intensity ) to 10-20 ms ( when the conditioning stimulus exceeded the test by up to 40 dB ) .
	manualset3
203613	5	417581	7	NULL	NULL	0	NULL	short interstimulus intervals	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	When the conditioning and test stimuli were of equal frequencies , the test response was markedly suppressed at short interstimulus intervals ; complete recovery appeared at intervals from about 2 ms ( when two stimuli were of equal intensity ) to 10-20 ms ( when the conditioning stimulus exceeded the test by up to 40 dB ) .
	manualset3
203614	6	417581	7	NULL	NULL	0	NULL	intervals	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	When the conditioning and test stimuli were of equal frequencies , the test response was markedly suppressed at short interstimulus intervals ; complete recovery appeared at intervals from about 2 ms ( when two stimuli were of equal intensity ) to 10-20 ms ( when the conditioning stimulus exceeded the test by up to 40 dB ) .
	manualset3
203615	7	417581	7	NULL	NULL	0	NULL	2 ms	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	When the conditioning and test stimuli were of equal frequencies , the test response was markedly suppressed at short interstimulus intervals ; complete recovery appeared at intervals from about 2 ms ( when two stimuli were of equal intensity ) to 10-20 ms ( when the conditioning stimulus exceeded the test by up to 40 dB ) .
	manualset3
203616	8	417581	7	NULL	NULL	0	NULL	two stimuli	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	When the conditioning and test stimuli were of equal frequencies , the test response was markedly suppressed at short interstimulus intervals ; complete recovery appeared at intervals from about 2 ms ( when two stimuli were of equal intensity ) to 10-20 ms ( when the conditioning stimulus exceeded the test by up to 40 dB ) .
	manualset3
203617	9	417581	7	NULL	NULL	NULL	NULL	 equal intensity	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When the conditioning and test stimuli were of equal frequencies , the test response was markedly suppressed at short interstimulus intervals ; complete recovery appeared at intervals from about 2 ms ( when two stimuli were of equal intensity ) to 10-20 ms ( when the conditioning stimulus exceeded the test by up to 40 dB ) .
	manualset3
203618	10	417581	7	NULL	NULL	0	NULL	 10-20 ms	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	When the conditioning and test stimuli were of equal frequencies , the test response was markedly suppressed at short interstimulus intervals ; complete recovery appeared at intervals from about 2 ms ( when two stimuli were of equal intensity ) to 10-20 ms ( when the conditioning stimulus exceeded the test by up to 40 dB ) .
	manualset3
203619	11	417581	7	NULL	NULL	0	NULL	conditioning stimulus	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	When the conditioning and test stimuli were of equal frequencies , the test response was markedly suppressed at short interstimulus intervals ; complete recovery appeared at intervals from about 2 ms ( when two stimuli were of equal intensity ) to 10-20 ms ( when the conditioning stimulus exceeded the test by up to 40 dB ) .
	manualset3
203620	12	417581	7	NULL	NULL	0	NULL	 test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	When the conditioning and test stimuli were of equal frequencies , the test response was markedly suppressed at short interstimulus intervals ; complete recovery appeared at intervals from about 2 ms ( when two stimuli were of equal intensity ) to 10-20 ms ( when the conditioning stimulus exceeded the test by up to 40 dB ) .
	manualset3
203621	13	417581	7	NULL	NULL	0	NULL	40 dB	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When the conditioning and test stimuli were of equal frequencies , the test response was markedly suppressed at short interstimulus intervals ; complete recovery appeared at intervals from about 2 ms ( when two stimuli were of equal intensity ) to 10-20 ms ( when the conditioning stimulus exceeded the test by up to 40 dB ) .
	manualset3
205513	14	417581	7	NULL	NULL	0	NULL	complete recovery	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When the conditioning and test stimuli were of equal frequencies , the test response was markedly suppressed at short interstimulus intervals ; complete recovery appeared at intervals from about 2 ms ( when two stimuli were of equal intensity ) to 10-20 ms ( when the conditioning stimulus exceeded the test by up to 40 dB ) .
	manualset3
203622	1	417582	7	NULL	NULL	0	NULL	early disappearance rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When the early disappearance rates ( 10 min ) of either total serum radioactivity or specifically the chylomicron fraction were compared , there were no differences between the groups receiving OA - or EPA-enriched chylomicrons .
	manualset3
203623	2	417582	7	NULL	NULL	0	NULL	10 min 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	When the early disappearance rates ( 10 min ) of either total serum radioactivity or specifically the chylomicron fraction were compared , there were no differences between the groups receiving OA - or EPA-enriched chylomicrons .
	manualset3
203624	3	417582	7	NULL	NULL	NULL	NULL	total serum radioactivity	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When the early disappearance rates ( 10 min ) of either total serum radioactivity or specifically the chylomicron fraction were compared , there were no differences between the groups receiving OA - or EPA-enriched chylomicrons .
	manualset3
203625	4	417582	7	NULL	NULL	0	NULL	chylomicron fraction	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When the early disappearance rates ( 10 min ) of either total serum radioactivity or specifically the chylomicron fraction were compared , there were no differences between the groups receiving OA - or EPA-enriched chylomicrons .
	manualset3
203626	5	417582	7	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	When the early disappearance rates ( 10 min ) of either total serum radioactivity or specifically the chylomicron fraction were compared , there were no differences between the groups receiving OA - or EPA-enriched chylomicrons .
	manualset3
203627	6	417582	7	NULL	NULL	0	NULL	groups 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When the early disappearance rates ( 10 min ) of either total serum radioactivity or specifically the chylomicron fraction were compared , there were no differences between the groups receiving OA - or EPA-enriched chylomicrons .
	manualset3
203628	7	417582	7	NULL	NULL	0	NULL	OA -enriched chylomicrons	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When the early disappearance rates ( 10 min ) of either total serum radioactivity or specifically the chylomicron fraction were compared , there were no differences between the groups receiving OA - or EPA-enriched chylomicrons .
	manualset3
203629	8	417582	7	NULL	NULL	0	NULL	EPA-enriched chylomicrons	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When the early disappearance rates ( 10 min ) of either total serum radioactivity or specifically the chylomicron fraction were compared , there were no differences between the groups receiving OA - or EPA-enriched chylomicrons .
	manualset3
203630	1	417583	7	NULL	NULL	0	NULL	 participants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All participants had heard of superinfection and one-third considered it a personal risk when they had UAI with men with the same sero-status .
	manualset3
203631	2	417583	7	NULL	NULL	0	NULL	superinfection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All participants had heard of superinfection and one-third considered it a personal risk when they had UAI with men with the same sero-status .
	manualset3
203632	3	417583	7	NULL	NULL	0	NULL	one-third	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All participants had heard of superinfection and one-third considered it a personal risk when they had UAI with men with the same sero-status .
	manualset3
203633	4	417583	7	NULL	NULL	0	NULL	personal risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All participants had heard of superinfection and one-third considered it a personal risk when they had UAI with men with the same sero-status .
	manualset3
203634	5	417583	7	NULL	NULL	NULL	NULL	UAI	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	All participants had heard of superinfection and one-third considered it a personal risk when they had UAI with men with the same sero-status .
	manualset3
203635	6	417583	7	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All participants had heard of superinfection and one-third considered it a personal risk when they had UAI with men with the same sero-status .
	manualset3
203636	7	417583	7	NULL	NULL	0	NULL	sero-status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All participants had heard of superinfection and one-third considered it a personal risk when they had UAI with men with the same sero-status .
	manualset3
203637	1	417584	7	NULL	NULL	0	NULL	 entire FCT type 1 pilus region	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When the entire FCT type 1 pilus region was ectopically expressed in serotype M1 strain SF370 , biofilm formation was promoted and autoaggregation was inhibited .
	manualset3
203638	2	417584	7	NULL	NULL	0	NULL	serotype M1 strain SF370	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When the entire FCT type 1 pilus region was ectopically expressed in serotype M1 strain SF370 , biofilm formation was promoted and autoaggregation was inhibited .
	manualset3
203639	3	417584	7	NULL	NULL	0	NULL	biofilm formation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When the entire FCT type 1 pilus region was ectopically expressed in serotype M1 strain SF370 , biofilm formation was promoted and autoaggregation was inhibited .
	manualset3
203640	4	417584	7	NULL	NULL	0	NULL	autoaggregation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When the entire FCT type 1 pilus region was ectopically expressed in serotype M1 strain SF370 , biofilm formation was promoted and autoaggregation was inhibited .
	manualset3
203641	1	417585	7	NULL	NULL	0	NULL	sites of formation	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When the known sites of formation of GI hormones were removed by resection of antrum , duodenum , pancreas , jejunum , ileum , and colon , the gastric stimulatory effect of amino acids was not changed significantly in denervated stomachs but was greatly increased in innervated stomachs .
	manualset3
203642	2	417585	7	NULL	NULL	0	NULL	GI hormones	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When the known sites of formation of GI hormones were removed by resection of antrum , duodenum , pancreas , jejunum , ileum , and colon , the gastric stimulatory effect of amino acids was not changed significantly in denervated stomachs but was greatly increased in innervated stomachs .
	manualset3
203643	3	417585	7	NULL	NULL	0	NULL	resection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	When the known sites of formation of GI hormones were removed by resection of antrum , duodenum , pancreas , jejunum , ileum , and colon , the gastric stimulatory effect of amino acids was not changed significantly in denervated stomachs but was greatly increased in innervated stomachs .
	manualset3
203644	4	417585	7	NULL	NULL	0	NULL	antrum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When the known sites of formation of GI hormones were removed by resection of antrum , duodenum , pancreas , jejunum , ileum , and colon , the gastric stimulatory effect of amino acids was not changed significantly in denervated stomachs but was greatly increased in innervated stomachs .
	manualset3
203645	5	417585	7	NULL	NULL	0	NULL	duodenum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When the known sites of formation of GI hormones were removed by resection of antrum , duodenum , pancreas , jejunum , ileum , and colon , the gastric stimulatory effect of amino acids was not changed significantly in denervated stomachs but was greatly increased in innervated stomachs .
	manualset3
203646	6	417585	7	NULL	NULL	0	NULL	pancreas 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When the known sites of formation of GI hormones were removed by resection of antrum , duodenum , pancreas , jejunum , ileum , and colon , the gastric stimulatory effect of amino acids was not changed significantly in denervated stomachs but was greatly increased in innervated stomachs .
	manualset3
203647	7	417585	7	NULL	NULL	0	NULL	 jejunum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When the known sites of formation of GI hormones were removed by resection of antrum , duodenum , pancreas , jejunum , ileum , and colon , the gastric stimulatory effect of amino acids was not changed significantly in denervated stomachs but was greatly increased in innervated stomachs .
	manualset3
203648	8	417585	7	NULL	NULL	0	NULL	ileum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When the known sites of formation of GI hormones were removed by resection of antrum , duodenum , pancreas , jejunum , ileum , and colon , the gastric stimulatory effect of amino acids was not changed significantly in denervated stomachs but was greatly increased in innervated stomachs .
	manualset3
203649	9	417585	7	NULL	NULL	0	NULL	colon	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When the known sites of formation of GI hormones were removed by resection of antrum , duodenum , pancreas , jejunum , ileum , and colon , the gastric stimulatory effect of amino acids was not changed significantly in denervated stomachs but was greatly increased in innervated stomachs .
	manualset3
203650	10	417585	7	NULL	NULL	0	NULL	 gastric stimulatory effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When the known sites of formation of GI hormones were removed by resection of antrum , duodenum , pancreas , jejunum , ileum , and colon , the gastric stimulatory effect of amino acids was not changed significantly in denervated stomachs but was greatly increased in innervated stomachs .
	manualset3
203651	11	417585	7	NULL	NULL	0	NULL	amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	When the known sites of formation of GI hormones were removed by resection of antrum , duodenum , pancreas , jejunum , ileum , and colon , the gastric stimulatory effect of amino acids was not changed significantly in denervated stomachs but was greatly increased in innervated stomachs .
	manualset3
203652	12	417585	7	NULL	NULL	0	NULL	denervated stomachs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When the known sites of formation of GI hormones were removed by resection of antrum , duodenum , pancreas , jejunum , ileum , and colon , the gastric stimulatory effect of amino acids was not changed significantly in denervated stomachs but was greatly increased in innervated stomachs .
	manualset3
203653	13	417585	7	NULL	NULL	0	NULL	 innervated stomachs 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When the known sites of formation of GI hormones were removed by resection of antrum , duodenum , pancreas , jejunum , ileum , and colon , the gastric stimulatory effect of amino acids was not changed significantly in denervated stomachs but was greatly increased in innervated stomachs .
	manualset3
203654	1	417586	7	NULL	NULL	0	NULL	partial pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When the partial pressure of arterial oxygen ( PaO ( 2 ) ) is ) or = 80 mmHg , it is unlikely that the patient has HPS .
	manualset3
203655	2	417586	7	NULL	NULL	0	NULL	arterial oxygen ( PaO ( 2 ) )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When the partial pressure of arterial oxygen ( PaO ( 2 ) ) is ) or = 80 mmHg , it is unlikely that the patient has HPS .
	manualset3
203656	3	417586	7	NULL	NULL	0	NULL	80 mmHg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	When the partial pressure of arterial oxygen ( PaO ( 2 ) ) is ) or = 80 mmHg , it is unlikely that the patient has HPS .
	manualset3
203657	4	417586	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	When the partial pressure of arterial oxygen ( PaO ( 2 ) ) is ) or = 80 mmHg , it is unlikely that the patient has HPS .
	manualset3
203658	5	417586	7	NULL	NULL	0	NULL	HPS	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	When the partial pressure of arterial oxygen ( PaO ( 2 ) ) is ) or = 80 mmHg , it is unlikely that the patient has HPS .
	manualset3
203659	1	417587	7	NULL	NULL	0	NULL	present findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When the present findings were combined with our previous results it turned out that AS , and psoriasis with or without arthropathy , and acute anterior uveitis ( AAU ) in combination with sacro-iliitis , may be described as IgA-related conditions and that increased serum C4 was related to sacro-iliitis in all these disorders .
	manualset3
203660	2	417587	7	NULL	NULL	0	NULL	previous results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When the present findings were combined with our previous results it turned out that AS , and psoriasis with or without arthropathy , and acute anterior uveitis ( AAU ) in combination with sacro-iliitis , may be described as IgA-related conditions and that increased serum C4 was related to sacro-iliitis in all these disorders .
	manualset3
203661	3	417587	7	NULL	NULL	0	NULL	AS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	When the present findings were combined with our previous results it turned out that AS , and psoriasis with or without arthropathy , and acute anterior uveitis ( AAU ) in combination with sacro-iliitis , may be described as IgA-related conditions and that increased serum C4 was related to sacro-iliitis in all these disorders .
	manualset3
203662	4	417587	7	NULL	NULL	0	NULL	psoriasis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	When the present findings were combined with our previous results it turned out that AS , and psoriasis with or without arthropathy , and acute anterior uveitis ( AAU ) in combination with sacro-iliitis , may be described as IgA-related conditions and that increased serum C4 was related to sacro-iliitis in all these disorders .
	manualset3
203663	5	417587	7	NULL	NULL	0	NULL	arthropathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	When the present findings were combined with our previous results it turned out that AS , and psoriasis with or without arthropathy , and acute anterior uveitis ( AAU ) in combination with sacro-iliitis , may be described as IgA-related conditions and that increased serum C4 was related to sacro-iliitis in all these disorders .
	manualset3
203664	6	417587	7	NULL	NULL	0	NULL	acute anterior uveitis ( AAU )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	When the present findings were combined with our previous results it turned out that AS , and psoriasis with or without arthropathy , and acute anterior uveitis ( AAU ) in combination with sacro-iliitis , may be described as IgA-related conditions and that increased serum C4 was related to sacro-iliitis in all these disorders .
	manualset3
203665	7	417587	7	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When the present findings were combined with our previous results it turned out that AS , and psoriasis with or without arthropathy , and acute anterior uveitis ( AAU ) in combination with sacro-iliitis , may be described as IgA-related conditions and that increased serum C4 was related to sacro-iliitis in all these disorders .
	manualset3
203666	8	417587	7	NULL	NULL	0	NULL	sacro-iliitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	When the present findings were combined with our previous results it turned out that AS , and psoriasis with or without arthropathy , and acute anterior uveitis ( AAU ) in combination with sacro-iliitis , may be described as IgA-related conditions and that increased serum C4 was related to sacro-iliitis in all these disorders .
	manualset3
203667	9	417587	7	NULL	NULL	0	NULL	IgA-related conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	When the present findings were combined with our previous results it turned out that AS , and psoriasis with or without arthropathy , and acute anterior uveitis ( AAU ) in combination with sacro-iliitis , may be described as IgA-related conditions and that increased serum C4 was related to sacro-iliitis in all these disorders .
	manualset3
203668	10	417587	7	NULL	NULL	0	NULL	increased serum C4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When the present findings were combined with our previous results it turned out that AS , and psoriasis with or without arthropathy , and acute anterior uveitis ( AAU ) in combination with sacro-iliitis , may be described as IgA-related conditions and that increased serum C4 was related to sacro-iliitis in all these disorders .
	manualset3
203669	11	417587	7	NULL	NULL	0	NULL	sacro-iliitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	When the present findings were combined with our previous results it turned out that AS , and psoriasis with or without arthropathy , and acute anterior uveitis ( AAU ) in combination with sacro-iliitis , may be described as IgA-related conditions and that increased serum C4 was related to sacro-iliitis in all these disorders .
	manualset3
203670	12	417587	7	NULL	NULL	0	NULL	disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	When the present findings were combined with our previous results it turned out that AS , and psoriasis with or without arthropathy , and acute anterior uveitis ( AAU ) in combination with sacro-iliitis , may be described as IgA-related conditions and that increased serum C4 was related to sacro-iliitis in all these disorders .
	manualset3
203716	1	417588	7	NULL	NULL	0	NULL	 propagation path	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When the propagation path is closed , modes consisting of one or several solitons may rotate around the ring , the topology of which imposes additional constraints on their allowed frequencies and phases .
	manualset3
203717	2	417588	7	NULL	NULL	0	NULL	modes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When the propagation path is closed , modes consisting of one or several solitons may rotate around the ring , the topology of which imposes additional constraints on their allowed frequencies and phases .
	manualset3
203718	3	417588	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When the propagation path is closed , modes consisting of one or several solitons may rotate around the ring , the topology of which imposes additional constraints on their allowed frequencies and phases .
	manualset3
203719	4	417588	7	NULL	NULL	0	NULL	solitons	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	When the propagation path is closed , modes consisting of one or several solitons may rotate around the ring , the topology of which imposes additional constraints on their allowed frequencies and phases .
	manualset3
203720	5	417588	7	NULL	NULL	0	NULL	 ring	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When the propagation path is closed , modes consisting of one or several solitons may rotate around the ring , the topology of which imposes additional constraints on their allowed frequencies and phases .
	manualset3
203721	6	417588	7	NULL	NULL	0	NULL	topology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When the propagation path is closed , modes consisting of one or several solitons may rotate around the ring , the topology of which imposes additional constraints on their allowed frequencies and phases .
	manualset3
203722	7	417588	7	NULL	NULL	0	NULL	additional constraints	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When the propagation path is closed , modes consisting of one or several solitons may rotate around the ring , the topology of which imposes additional constraints on their allowed frequencies and phases .
	manualset3
203723	8	417588	7	NULL	NULL	0	NULL	 frequencies 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When the propagation path is closed , modes consisting of one or several solitons may rotate around the ring , the topology of which imposes additional constraints on their allowed frequencies and phases .
	manualset3
203724	9	417588	7	NULL	NULL	0	NULL	phases	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When the propagation path is closed , modes consisting of one or several solitons may rotate around the ring , the topology of which imposes additional constraints on their allowed frequencies and phases .
	manualset3
203725	1	417589	7	NULL	NULL	0	NULL	responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When the responses are compared before and after separation of the blood supply of the carotid bodies from the CS region and when they are compared before and after inhibition of reflex systemic hypotension by ganglionic blockade , the observed responses were shown to be due solely to CS baroreceptor stimulation and not to alterations in carotid body blood flow or reflex changes in systemic cardiovascular variables .
	manualset3
203726	2	417589	7	NULL	NULL	NULL	NULL	separation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When the responses are compared before and after separation of the blood supply of the carotid bodies from the CS region and when they are compared before and after inhibition of reflex systemic hypotension by ganglionic blockade , the observed responses were shown to be due solely to CS baroreceptor stimulation and not to alterations in carotid body blood flow or reflex changes in systemic cardiovascular variables .
	manualset3
203727	3	417589	7	NULL	NULL	0	NULL	 blood supply	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When the responses are compared before and after separation of the blood supply of the carotid bodies from the CS region and when they are compared before and after inhibition of reflex systemic hypotension by ganglionic blockade , the observed responses were shown to be due solely to CS baroreceptor stimulation and not to alterations in carotid body blood flow or reflex changes in systemic cardiovascular variables .
	manualset3
203728	4	417589	7	NULL	NULL	0	NULL	carotid bodies	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When the responses are compared before and after separation of the blood supply of the carotid bodies from the CS region and when they are compared before and after inhibition of reflex systemic hypotension by ganglionic blockade , the observed responses were shown to be due solely to CS baroreceptor stimulation and not to alterations in carotid body blood flow or reflex changes in systemic cardiovascular variables .
	manualset3
203729	5	417589	7	NULL	NULL	0	NULL	CS region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When the responses are compared before and after separation of the blood supply of the carotid bodies from the CS region and when they are compared before and after inhibition of reflex systemic hypotension by ganglionic blockade , the observed responses were shown to be due solely to CS baroreceptor stimulation and not to alterations in carotid body blood flow or reflex changes in systemic cardiovascular variables .
	manualset3
203730	6	417589	7	NULL	NULL	NULL	NULL	inhibition 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When the responses are compared before and after separation of the blood supply of the carotid bodies from the CS region and when they are compared before and after inhibition of reflex systemic hypotension by ganglionic blockade , the observed responses were shown to be due solely to CS baroreceptor stimulation and not to alterations in carotid body blood flow or reflex changes in systemic cardiovascular variables .
	manualset3
203731	7	417589	7	NULL	NULL	NULL	NULL	reflex systemic hypotension	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When the responses are compared before and after separation of the blood supply of the carotid bodies from the CS region and when they are compared before and after inhibition of reflex systemic hypotension by ganglionic blockade , the observed responses were shown to be due solely to CS baroreceptor stimulation and not to alterations in carotid body blood flow or reflex changes in systemic cardiovascular variables .
	manualset3
203732	8	417589	7	NULL	NULL	0	NULL	ganglionic blockade	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When the responses are compared before and after separation of the blood supply of the carotid bodies from the CS region and when they are compared before and after inhibition of reflex systemic hypotension by ganglionic blockade , the observed responses were shown to be due solely to CS baroreceptor stimulation and not to alterations in carotid body blood flow or reflex changes in systemic cardiovascular variables .
	manualset3
203733	9	417589	7	NULL	NULL	0	NULL	observed responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When the responses are compared before and after separation of the blood supply of the carotid bodies from the CS region and when they are compared before and after inhibition of reflex systemic hypotension by ganglionic blockade , the observed responses were shown to be due solely to CS baroreceptor stimulation and not to alterations in carotid body blood flow or reflex changes in systemic cardiovascular variables .
	manualset3
203734	10	417589	7	NULL	NULL	NULL	NULL	CS baroreceptor stimulation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When the responses are compared before and after separation of the blood supply of the carotid bodies from the CS region and when they are compared before and after inhibition of reflex systemic hypotension by ganglionic blockade , the observed responses were shown to be due solely to CS baroreceptor stimulation and not to alterations in carotid body blood flow or reflex changes in systemic cardiovascular variables .
	manualset3
203735	11	417589	7	NULL	NULL	0	NULL	alterations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When the responses are compared before and after separation of the blood supply of the carotid bodies from the CS region and when they are compared before and after inhibition of reflex systemic hypotension by ganglionic blockade , the observed responses were shown to be due solely to CS baroreceptor stimulation and not to alterations in carotid body blood flow or reflex changes in systemic cardiovascular variables .
	manualset3
203736	12	417589	7	NULL	NULL	0	NULL	carotid body blood flow	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When the responses are compared before and after separation of the blood supply of the carotid bodies from the CS region and when they are compared before and after inhibition of reflex systemic hypotension by ganglionic blockade , the observed responses were shown to be due solely to CS baroreceptor stimulation and not to alterations in carotid body blood flow or reflex changes in systemic cardiovascular variables .
	manualset3
203737	13	417589	7	NULL	NULL	0	NULL	reflex changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When the responses are compared before and after separation of the blood supply of the carotid bodies from the CS region and when they are compared before and after inhibition of reflex systemic hypotension by ganglionic blockade , the observed responses were shown to be due solely to CS baroreceptor stimulation and not to alterations in carotid body blood flow or reflex changes in systemic cardiovascular variables .
	manualset3
203738	14	417589	7	NULL	NULL	0	NULL	systemic cardiovascular variables 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When the responses are compared before and after separation of the blood supply of the carotid bodies from the CS region and when they are compared before and after inhibition of reflex systemic hypotension by ganglionic blockade , the observed responses were shown to be due solely to CS baroreceptor stimulation and not to alterations in carotid body blood flow or reflex changes in systemic cardiovascular variables .
	manualset3
203747	1	417590	7	NULL	NULL	0	NULL	shield rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When the shield rate was 0 % , a hyperechoic region occurred , even when a maximum sonication power was not used .
	manualset3
203748	2	417590	7	NULL	NULL	0	NULL	0 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When the shield rate was 0 % , a hyperechoic region occurred , even when a maximum sonication power was not used .
	manualset3
203749	3	417590	7	NULL	NULL	0	NULL	 hyperechoic region	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When the shield rate was 0 % , a hyperechoic region occurred , even when a maximum sonication power was not used .
	manualset3
203750	4	417590	7	NULL	NULL	0	NULL	maximum sonication power	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	When the shield rate was 0 % , a hyperechoic region occurred , even when a maximum sonication power was not used .
	manualset3
203751	1	417591	7	NULL	NULL	0	NULL	transmembrane electrical potential 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When the transmembrane electrical potential is lowered by isotonic replacement of Na with K , this neither by itself stimulates proliferation nor does it inhibit mitogen-stimulated proliferation .
	manualset3
203752	2	417591	7	NULL	NULL	0	NULL	 isotonic replacement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When the transmembrane electrical potential is lowered by isotonic replacement of Na with K , this neither by itself stimulates proliferation nor does it inhibit mitogen-stimulated proliferation .
	manualset3
203753	3	417591	7	NULL	NULL	0	NULL	Na	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When the transmembrane electrical potential is lowered by isotonic replacement of Na with K , this neither by itself stimulates proliferation nor does it inhibit mitogen-stimulated proliferation .
	manualset3
203754	4	417591	7	NULL	NULL	0	NULL	 K	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When the transmembrane electrical potential is lowered by isotonic replacement of Na with K , this neither by itself stimulates proliferation nor does it inhibit mitogen-stimulated proliferation .
	manualset3
203755	5	417591	7	NULL	NULL	0	NULL	proliferation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When the transmembrane electrical potential is lowered by isotonic replacement of Na with K , this neither by itself stimulates proliferation nor does it inhibit mitogen-stimulated proliferation .
	manualset3
203756	6	417591	7	NULL	NULL	0	NULL	mitogen-stimulated proliferation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When the transmembrane electrical potential is lowered by isotonic replacement of Na with K , this neither by itself stimulates proliferation nor does it inhibit mitogen-stimulated proliferation .
	manualset3
203762	1	417592	7	NULL	NULL	0	NULL	 transplants	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When the transplants were exposed to gestational hormonal milieu , few or no fibers were observed to the end of pregnancy ; however , a significant increase at post partum was observed .
	manualset3
203763	2	417592	7	NULL	NULL	0	NULL	gestational hormonal milieu	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When the transplants were exposed to gestational hormonal milieu , few or no fibers were observed to the end of pregnancy ; however , a significant increase at post partum was observed .
	manualset3
203766	3	417592	7	NULL	NULL	NULL	NULL	fibers	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When the transplants were exposed to gestational hormonal milieu , few or no fibers were observed to the end of pregnancy ; however , a significant increase at post partum was observed .
	manualset3
203767	4	417592	7	NULL	NULL	0	NULL	end 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When the transplants were exposed to gestational hormonal milieu , few or no fibers were observed to the end of pregnancy ; however , a significant increase at post partum was observed .
	manualset3
203768	5	417592	7	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When the transplants were exposed to gestational hormonal milieu , few or no fibers were observed to the end of pregnancy ; however , a significant increase at post partum was observed .
	manualset3
203769	6	417592	7	NULL	NULL	0	NULL	significant increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When the transplants were exposed to gestational hormonal milieu , few or no fibers were observed to the end of pregnancy ; however , a significant increase at post partum was observed .
	manualset3
203770	7	417592	7	NULL	NULL	0	NULL	post partum 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When the transplants were exposed to gestational hormonal milieu , few or no fibers were observed to the end of pregnancy ; however , a significant increase at post partum was observed .
	manualset3
203771	1	417593	7	NULL	NULL	0	NULL	transport system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When the transport system is inhibited to 50-60 % by butanedione , the transporter can still bind covalently the anion transport inhibitor 2H2DIDS up to 85 + / - 12 % of its total binding capacity .
	manualset3
203772	2	417593	7	NULL	NULL	0	NULL	 50-60 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When the transport system is inhibited to 50-60 % by butanedione , the transporter can still bind covalently the anion transport inhibitor 2H2DIDS up to 85 + / - 12 % of its total binding capacity .
	manualset3
203773	3	417593	7	NULL	NULL	0	NULL	butanedione	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When the transport system is inhibited to 50-60 % by butanedione , the transporter can still bind covalently the anion transport inhibitor 2H2DIDS up to 85 + / - 12 % of its total binding capacity .
	manualset3
203774	4	417593	7	NULL	NULL	0	NULL	transporter	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When the transport system is inhibited to 50-60 % by butanedione , the transporter can still bind covalently the anion transport inhibitor 2H2DIDS up to 85 + / - 12 % of its total binding capacity .
	manualset3
203775	5	417593	7	NULL	NULL	0	NULL	anion transport inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When the transport system is inhibited to 50-60 % by butanedione , the transporter can still bind covalently the anion transport inhibitor 2H2DIDS up to 85 + / - 12 % of its total binding capacity .
	manualset3
203776	6	417593	7	NULL	NULL	0	NULL	2H2DIDS	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When the transport system is inhibited to 50-60 % by butanedione , the transporter can still bind covalently the anion transport inhibitor 2H2DIDS up to 85 + / - 12 % of its total binding capacity .
	manualset3
203777	7	417593	7	NULL	NULL	0	NULL	85 + / - 12 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When the transport system is inhibited to 50-60 % by butanedione , the transporter can still bind covalently the anion transport inhibitor 2H2DIDS up to 85 + / - 12 % of its total binding capacity .
	manualset3
203778	8	417593	7	NULL	NULL	0	NULL	total binding capacity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When the transport system is inhibited to 50-60 % by butanedione , the transporter can still bind covalently the anion transport inhibitor 2H2DIDS up to 85 + / - 12 % of its total binding capacity .
	manualset3
203781	1	417594	7	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	When the treatment was extended for 60 days , spermatogenic arrest and loss of libido were evident in animals treated with 5 mg dose ; animals receiving 1 mg dose of steroid showed no decrease of spermatogenesis or sexual activity and their fertility remained unaffected .
	manualset3
203783	2	417594	7	NULL	NULL	0	NULL	60 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	When the treatment was extended for 60 days , spermatogenic arrest and loss of libido were evident in animals treated with 5 mg dose ; animals receiving 1 mg dose of steroid showed no decrease of spermatogenesis or sexual activity and their fertility remained unaffected .
	manualset3
203786	3	417594	7	NULL	NULL	0	NULL	spermatogenic arrest	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When the treatment was extended for 60 days , spermatogenic arrest and loss of libido were evident in animals treated with 5 mg dose ; animals receiving 1 mg dose of steroid showed no decrease of spermatogenesis or sexual activity and their fertility remained unaffected .
	manualset3
203788	4	417594	7	NULL	NULL	0	NULL	 loss of libido	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When the treatment was extended for 60 days , spermatogenic arrest and loss of libido were evident in animals treated with 5 mg dose ; animals receiving 1 mg dose of steroid showed no decrease of spermatogenesis or sexual activity and their fertility remained unaffected .
	manualset3
203790	5	417594	7	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When the treatment was extended for 60 days , spermatogenic arrest and loss of libido were evident in animals treated with 5 mg dose ; animals receiving 1 mg dose of steroid showed no decrease of spermatogenesis or sexual activity and their fertility remained unaffected .
	manualset3
203791	6	417594	7	NULL	NULL	0	NULL	5 mg dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When the treatment was extended for 60 days , spermatogenic arrest and loss of libido were evident in animals treated with 5 mg dose ; animals receiving 1 mg dose of steroid showed no decrease of spermatogenesis or sexual activity and their fertility remained unaffected .
	manualset3
203792	7	417594	7	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When the treatment was extended for 60 days , spermatogenic arrest and loss of libido were evident in animals treated with 5 mg dose ; animals receiving 1 mg dose of steroid showed no decrease of spermatogenesis or sexual activity and their fertility remained unaffected .
	manualset3
203793	8	417594	7	NULL	NULL	0	NULL	1 mg dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When the treatment was extended for 60 days , spermatogenic arrest and loss of libido were evident in animals treated with 5 mg dose ; animals receiving 1 mg dose of steroid showed no decrease of spermatogenesis or sexual activity and their fertility remained unaffected .
	manualset3
203794	9	417594	7	NULL	NULL	0	NULL	steroid 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	When the treatment was extended for 60 days , spermatogenic arrest and loss of libido were evident in animals treated with 5 mg dose ; animals receiving 1 mg dose of steroid showed no decrease of spermatogenesis or sexual activity and their fertility remained unaffected .
	manualset3
203801	10	417594	7	NULL	NULL	0	NULL	no decrease	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When the treatment was extended for 60 days , spermatogenic arrest and loss of libido were evident in animals treated with 5 mg dose ; animals receiving 1 mg dose of steroid showed no decrease of spermatogenesis or sexual activity and their fertility remained unaffected .
	manualset3
203806	11	417594	7	NULL	NULL	0	NULL	spermatogenesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When the treatment was extended for 60 days , spermatogenic arrest and loss of libido were evident in animals treated with 5 mg dose ; animals receiving 1 mg dose of steroid showed no decrease of spermatogenesis or sexual activity and their fertility remained unaffected .
	manualset3
203807	12	417594	7	NULL	NULL	0	NULL	sexual activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When the treatment was extended for 60 days , spermatogenic arrest and loss of libido were evident in animals treated with 5 mg dose ; animals receiving 1 mg dose of steroid showed no decrease of spermatogenesis or sexual activity and their fertility remained unaffected .
	manualset3
203808	13	417594	7	NULL	NULL	0	NULL	fertility	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When the treatment was extended for 60 days , spermatogenic arrest and loss of libido were evident in animals treated with 5 mg dose ; animals receiving 1 mg dose of steroid showed no decrease of spermatogenesis or sexual activity and their fertility remained unaffected .
	manualset3
203816	1	417595	7	NULL	NULL	0	NULL	 cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	When these cells were simultaneously infected with HSV-1 KOS and HSV-2 186 , HSV-1 KOS interfered with the rapid suppression of globin synthesis induced by HSV-2 186 .
	manualset3
203818	2	417595	7	NULL	NULL	0	NULL	HSV-1 KOS	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When these cells were simultaneously infected with HSV-1 KOS and HSV-2 186 , HSV-1 KOS interfered with the rapid suppression of globin synthesis induced by HSV-2 186 .
	manualset3
203820	3	417595	7	NULL	NULL	0	NULL	HSV-2 186	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When these cells were simultaneously infected with HSV-1 KOS and HSV-2 186 , HSV-1 KOS interfered with the rapid suppression of globin synthesis induced by HSV-2 186 .
	manualset3
203822	4	417595	7	NULL	NULL	0	NULL	HSV-1 KOS	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When these cells were simultaneously infected with HSV-1 KOS and HSV-2 186 , HSV-1 KOS interfered with the rapid suppression of globin synthesis induced by HSV-2 186 .
	manualset3
203826	5	417595	7	NULL	NULL	0	NULL	rapid suppression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When these cells were simultaneously infected with HSV-1 KOS and HSV-2 186 , HSV-1 KOS interfered with the rapid suppression of globin synthesis induced by HSV-2 186 .
	manualset3
203828	6	417595	7	NULL	NULL	0	NULL	globin synthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When these cells were simultaneously infected with HSV-1 KOS and HSV-2 186 , HSV-1 KOS interfered with the rapid suppression of globin synthesis induced by HSV-2 186 .
	manualset3
203831	7	417595	7	NULL	NULL	0	NULL	HSV-2 186	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When these cells were simultaneously infected with HSV-1 KOS and HSV-2 186 , HSV-1 KOS interfered with the rapid suppression of globin synthesis induced by HSV-2 186 .
	manualset3
203833	1	417596	7	NULL	NULL	0	NULL	stoichiometric studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	When these stoichiometric studies were performed with cell-bound IgE , it was found that only one of the sites recognized by 51.3 mAb was involved in the Fc epsilon R binding site .
	manualset3
203834	2	417596	7	NULL	NULL	0	NULL	cell-bound IgE	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When these stoichiometric studies were performed with cell-bound IgE , it was found that only one of the sites recognized by 51.3 mAb was involved in the Fc epsilon R binding site .
	manualset3
203835	3	417596	7	NULL	NULL	0	NULL	one of the sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	When these stoichiometric studies were performed with cell-bound IgE , it was found that only one of the sites recognized by 51.3 mAb was involved in the Fc epsilon R binding site .
	manualset3
203837	4	417596	7	NULL	NULL	0	NULL	51.3 mAb	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When these stoichiometric studies were performed with cell-bound IgE , it was found that only one of the sites recognized by 51.3 mAb was involved in the Fc epsilon R binding site .
	manualset3
203839	5	417596	7	NULL	NULL	0	NULL	Fc epsilon R binding site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	When these stoichiometric studies were performed with cell-bound IgE , it was found that only one of the sites recognized by 51.3 mAb was involved in the Fc epsilon R binding site .
	manualset3
203858	1	417597	7	NULL	NULL	0	NULL	tubules	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When these tubules are returned to isotonic media , they immediately shrink to 78 % of control volume before showing evidence of VRI .
	manualset3
203862	2	417597	7	NULL	NULL	0	NULL	isotonic media	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When these tubules are returned to isotonic media , they immediately shrink to 78 % of control volume before showing evidence of VRI .
	manualset3
203863	3	417597	7	NULL	NULL	0	NULL	 78 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When these tubules are returned to isotonic media , they immediately shrink to 78 % of control volume before showing evidence of VRI .
	manualset3
203864	4	417597	7	NULL	NULL	0	NULL	control volume 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When these tubules are returned to isotonic media , they immediately shrink to 78 % of control volume before showing evidence of VRI .
	manualset3
203865	5	417597	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When these tubules are returned to isotonic media , they immediately shrink to 78 % of control volume before showing evidence of VRI .
	manualset3
203866	6	417597	7	NULL	NULL	0	NULL	VRI .	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When these tubules are returned to isotonic media , they immediately shrink to 78 % of control volume before showing evidence of VRI .
	manualset3
203870	1	417598	7	NULL	NULL	0	NULL	genotype A	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	When they were superinfected with genotype A at week 10 , however , HBV DNA of genotype A developed , which was replaced almost completely by that of genotype G within 10 weeks .
	manualset3
203871	2	417598	7	NULL	NULL	NULL	NULL	week 10	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When they were superinfected with genotype A at week 10 , however , HBV DNA of genotype A developed , which was replaced almost completely by that of genotype G within 10 weeks .
	manualset3
203872	3	417598	7	NULL	NULL	0	NULL	HBV DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	When they were superinfected with genotype A at week 10 , however , HBV DNA of genotype A developed , which was replaced almost completely by that of genotype G within 10 weeks .
	manualset3
203873	4	417598	7	NULL	NULL	0	NULL	genotype A	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	When they were superinfected with genotype A at week 10 , however , HBV DNA of genotype A developed , which was replaced almost completely by that of genotype G within 10 weeks .
	manualset3
203874	5	417598	7	NULL	NULL	0	NULL	 genotype G	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	When they were superinfected with genotype A at week 10 , however , HBV DNA of genotype A developed , which was replaced almost completely by that of genotype G within 10 weeks .
	manualset3
203875	6	417598	7	NULL	NULL	0	NULL	10 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	When they were superinfected with genotype A at week 10 , however , HBV DNA of genotype A developed , which was replaced almost completely by that of genotype G within 10 weeks .
	manualset3
203876	1	417599	7	NULL	NULL	0	NULL	three subunits	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	When three subunits were expressed , alpha delta beta and alpha gamma beta complexes were formed .
	manualset3
203877	2	417599	7	NULL	NULL	0	NULL	alpha delta beta complexes	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	When three subunits were expressed , alpha delta beta and alpha gamma beta complexes were formed .
	manualset3
203878	3	417599	7	NULL	NULL	0	NULL	alpha gamma beta complexes	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	When three subunits were expressed , alpha delta beta and alpha gamma beta complexes were formed .
	manualset3
203880	1	417600	7	NULL	NULL	NULL	NULL	time of injury	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When treated at the time of injury with PRL levels of 62.5-1000 ng/mL , cells at the wound front became abnormal in shape and had reductions in f-actin staining in comparison to controls that were not PRL-treated .
	manualset3
203882	3	417600	7	NULL	NULL	0	NULL	PRL levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When treated at the time of injury with PRL levels of 62.5-1000 ng/mL , cells at the wound front became abnormal in shape and had reductions in f-actin staining in comparison to controls that were not PRL-treated .
	manualset3
203883	4	417600	7	NULL	NULL	0	NULL	62.5-1000 ng/mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	When treated at the time of injury with PRL levels of 62.5-1000 ng/mL , cells at the wound front became abnormal in shape and had reductions in f-actin staining in comparison to controls that were not PRL-treated .
	manualset3
203884	5	417600	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	When treated at the time of injury with PRL levels of 62.5-1000 ng/mL , cells at the wound front became abnormal in shape and had reductions in f-actin staining in comparison to controls that were not PRL-treated .
	manualset3
203886	6	417600	7	NULL	NULL	0	NULL	 wound front	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When treated at the time of injury with PRL levels of 62.5-1000 ng/mL , cells at the wound front became abnormal in shape and had reductions in f-actin staining in comparison to controls that were not PRL-treated .
	manualset3
203889	7	417600	7	NULL	NULL	0	NULL	shape	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When treated at the time of injury with PRL levels of 62.5-1000 ng/mL , cells at the wound front became abnormal in shape and had reductions in f-actin staining in comparison to controls that were not PRL-treated .
	manualset3
203891	8	417600	7	NULL	NULL	0	NULL	reductions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When treated at the time of injury with PRL levels of 62.5-1000 ng/mL , cells at the wound front became abnormal in shape and had reductions in f-actin staining in comparison to controls that were not PRL-treated .
	manualset3
203892	9	417600	7	NULL	NULL	0	NULL	f-actin staining	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When treated at the time of injury with PRL levels of 62.5-1000 ng/mL , cells at the wound front became abnormal in shape and had reductions in f-actin staining in comparison to controls that were not PRL-treated .
	manualset3
203893	10	417600	7	NULL	NULL	0	NULL	 comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	When treated at the time of injury with PRL levels of 62.5-1000 ng/mL , cells at the wound front became abnormal in shape and had reductions in f-actin staining in comparison to controls that were not PRL-treated .
	manualset3
205514	11	417600	7	NULL	NULL	NULL	NULL	controls	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When treated at the time of injury with PRL levels of 62.5-1000 ng/mL , cells at the wound front became abnormal in shape and had reductions in f-actin staining in comparison to controls that were not PRL-treated .
	manualset3
203896	1	417601	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients continued on rFVIII-BHK therapy , and all tested negative for inhibitors at the time of their last inhibitor assay during the observation period .
	manualset3
203899	2	417601	7	NULL	NULL	0	NULL	rFVIII-BHK therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients continued on rFVIII-BHK therapy , and all tested negative for inhibitors at the time of their last inhibitor assay during the observation period .
	manualset3
203901	3	417601	7	NULL	NULL	0	NULL	inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients continued on rFVIII-BHK therapy , and all tested negative for inhibitors at the time of their last inhibitor assay during the observation period .
	manualset3
203904	4	417601	7	NULL	NULL	0	NULL	 time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients continued on rFVIII-BHK therapy , and all tested negative for inhibitors at the time of their last inhibitor assay during the observation period .
	manualset3
203905	5	417601	7	NULL	NULL	0	NULL	inhibitor assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients continued on rFVIII-BHK therapy , and all tested negative for inhibitors at the time of their last inhibitor assay during the observation period .
	manualset3
203906	6	417601	7	NULL	NULL	0	NULL	observation period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients continued on rFVIII-BHK therapy , and all tested negative for inhibitors at the time of their last inhibitor assay during the observation period .
	manualset3
205515	7	417601	7	NULL	NULL	0	NULL	negative	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients continued on rFVIII-BHK therapy , and all tested negative for inhibitors at the time of their last inhibitor assay during the observation period .
	manualset3
203911	1	417602	7	NULL	NULL	0	NULL	dithionite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When treated with dithionite at neutral pH , the recombinant hemoglobin from Synechocystis sp .
	manualset3
203913	2	417602	7	NULL	NULL	0	NULL	 neutral pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When treated with dithionite at neutral pH , the recombinant hemoglobin from Synechocystis sp .
	manualset3
203915	3	417602	7	NULL	NULL	0	NULL	recombinant hemoglobin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When treated with dithionite at neutral pH , the recombinant hemoglobin from Synechocystis sp .
	manualset3
203917	4	417602	7	NULL	NULL	0	NULL	Synechocystis sp	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When treated with dithionite at neutral pH , the recombinant hemoglobin from Synechocystis sp .
	manualset3
203945	1	417603	7	NULL	NULL	0	NULL	oxytocin	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	When treated with oxytocin , Sca-1 + cells expressed genes of cardiac transcription factors and contractile proteins and showed sarcomeric structure and spontaneous beating .
	manualset3
203946	2	417603	7	NULL	NULL	0	NULL	Sca-1 + cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	When treated with oxytocin , Sca-1 + cells expressed genes of cardiac transcription factors and contractile proteins and showed sarcomeric structure and spontaneous beating .
	manualset3
203947	3	417603	7	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When treated with oxytocin , Sca-1 + cells expressed genes of cardiac transcription factors and contractile proteins and showed sarcomeric structure and spontaneous beating .
	manualset3
203948	4	417603	7	NULL	NULL	0	NULL	cardiac transcription factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When treated with oxytocin , Sca-1 + cells expressed genes of cardiac transcription factors and contractile proteins and showed sarcomeric structure and spontaneous beating .
	manualset3
203949	5	417603	7	NULL	NULL	0	NULL	contractile proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When treated with oxytocin , Sca-1 + cells expressed genes of cardiac transcription factors and contractile proteins and showed sarcomeric structure and spontaneous beating .
	manualset3
203954	6	417603	7	NULL	NULL	0	NULL	sarcomeric structure 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When treated with oxytocin , Sca-1 + cells expressed genes of cardiac transcription factors and contractile proteins and showed sarcomeric structure and spontaneous beating .
	manualset3
203955	7	417603	7	NULL	NULL	0	NULL	spontaneous beating	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When treated with oxytocin , Sca-1 + cells expressed genes of cardiac transcription factors and contractile proteins and showed sarcomeric structure and spontaneous beating .
	manualset3
203956	1	417604	7	NULL	NULL	0	NULL	 tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When tumors were palpable , the mice were treated with melphalan at doses shown to be effective against the melphalan-sensitive subpopulations .
	manualset3
203957	2	417604	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When tumors were palpable , the mice were treated with melphalan at doses shown to be effective against the melphalan-sensitive subpopulations .
	manualset3
203958	3	417604	7	NULL	NULL	NULL	NULL	melphalan	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When tumors were palpable , the mice were treated with melphalan at doses shown to be effective against the melphalan-sensitive subpopulations .
	manualset3
203959	4	417604	7	NULL	NULL	0	NULL	doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When tumors were palpable , the mice were treated with melphalan at doses shown to be effective against the melphalan-sensitive subpopulations .
	manualset3
203960	5	417604	7	NULL	NULL	0	NULL	melphalan-sensitive subpopulations	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When tumors were palpable , the mice were treated with melphalan at doses shown to be effective against the melphalan-sensitive subpopulations .
	manualset3
203962	1	417605	7	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When two or more of these forms of variation are used to delimit `` new '' extant or fossil species , any decision arrived at might be construed as arbitrary .
	manualset3
203963	2	417605	7	NULL	NULL	0	NULL	forms of variation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When two or more of these forms of variation are used to delimit `` new '' extant or fossil species , any decision arrived at might be construed as arbitrary .
	manualset3
203964	3	417605	7	NULL	NULL	0	NULL	`` new '' extant	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When two or more of these forms of variation are used to delimit `` new '' extant or fossil species , any decision arrived at might be construed as arbitrary .
	manualset3
203965	4	417605	7	NULL	NULL	0	NULL	fossil species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When two or more of these forms of variation are used to delimit `` new '' extant or fossil species , any decision arrived at might be construed as arbitrary .
	manualset3
203966	5	417605	7	NULL	NULL	0	NULL	decision	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When two or more of these forms of variation are used to delimit `` new '' extant or fossil species , any decision arrived at might be construed as arbitrary .
	manualset3
203970	1	417606	7	NULL	NULL	0	NULL	GnRH antagonist-assisted reproduction protocol	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	When used as part of a GnRH antagonist-assisted reproduction protocol , corifollitropin alfa was generally well tolerated , with a tolerability profile similar to that of rFSH .
	manualset3
203972	2	417606	7	NULL	NULL	0	NULL	corifollitropin alfa	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	When used as part of a GnRH antagonist-assisted reproduction protocol , corifollitropin alfa was generally well tolerated , with a tolerability profile similar to that of rFSH .
	manualset3
203982	3	417606	7	NULL	NULL	0	NULL	tolerability profile	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When used as part of a GnRH antagonist-assisted reproduction protocol , corifollitropin alfa was generally well tolerated , with a tolerability profile similar to that of rFSH .
	manualset3
203985	4	417606	7	NULL	NULL	0	NULL	rFSH 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When used as part of a GnRH antagonist-assisted reproduction protocol , corifollitropin alfa was generally well tolerated , with a tolerability profile similar to that of rFSH .
	manualset3
203986	1	417607	7	NULL	NULL	0	NULL	concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When used at equivalent concentrations in vitro , IL-15 was more potent than IL-2 as a growth factor for CD56 + cells , as well as for CD16 + cells and also CD4 + and CD8 + T cells .
	manualset3
203988	2	417607	7	NULL	NULL	0	NULL	 IL-15	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When used at equivalent concentrations in vitro , IL-15 was more potent than IL-2 as a growth factor for CD56 + cells , as well as for CD16 + cells and also CD4 + and CD8 + T cells .
	manualset3
203990	3	417607	7	NULL	NULL	0	NULL	IL-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When used at equivalent concentrations in vitro , IL-15 was more potent than IL-2 as a growth factor for CD56 + cells , as well as for CD16 + cells and also CD4 + and CD8 + T cells .
	manualset3
203991	4	417607	7	NULL	NULL	0	NULL	growth factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When used at equivalent concentrations in vitro , IL-15 was more potent than IL-2 as a growth factor for CD56 + cells , as well as for CD16 + cells and also CD4 + and CD8 + T cells .
	manualset3
203993	5	417607	7	NULL	NULL	0	NULL	 CD56 + cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	When used at equivalent concentrations in vitro , IL-15 was more potent than IL-2 as a growth factor for CD56 + cells , as well as for CD16 + cells and also CD4 + and CD8 + T cells .
	manualset3
203995	6	417607	7	NULL	NULL	0	NULL	 CD16 + cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	When used at equivalent concentrations in vitro , IL-15 was more potent than IL-2 as a growth factor for CD56 + cells , as well as for CD16 + cells and also CD4 + and CD8 + T cells .
	manualset3
203998	7	417607	7	NULL	NULL	0	NULL	CD4 + T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	When used at equivalent concentrations in vitro , IL-15 was more potent than IL-2 as a growth factor for CD56 + cells , as well as for CD16 + cells and also CD4 + and CD8 + T cells .
	manualset3
204001	8	417607	7	NULL	NULL	0	NULL	CD8 + T cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	When used at equivalent concentrations in vitro , IL-15 was more potent than IL-2 as a growth factor for CD56 + cells , as well as for CD16 + cells and also CD4 + and CD8 + T cells .
	manualset3
204002	1	417608	7	NULL	NULL	0	NULL	concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When we studied the concentration of lithium needed to inhibit phosphoglucomutase activity by 50 % , a bimodal distribution among the population tested was obtained .
	manualset3
204003	2	417608	7	NULL	NULL	0	NULL	 lithium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When we studied the concentration of lithium needed to inhibit phosphoglucomutase activity by 50 % , a bimodal distribution among the population tested was obtained .
	manualset3
204004	3	417608	7	NULL	NULL	0	NULL	phosphoglucomutase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When we studied the concentration of lithium needed to inhibit phosphoglucomutase activity by 50 % , a bimodal distribution among the population tested was obtained .
	manualset3
204005	4	417608	7	NULL	NULL	0	NULL	50 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When we studied the concentration of lithium needed to inhibit phosphoglucomutase activity by 50 % , a bimodal distribution among the population tested was obtained .
	manualset3
204006	5	417608	7	NULL	NULL	0	NULL	bimodal distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When we studied the concentration of lithium needed to inhibit phosphoglucomutase activity by 50 % , a bimodal distribution among the population tested was obtained .
	manualset3
204007	6	417608	7	NULL	NULL	0	NULL	population 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When we studied the concentration of lithium needed to inhibit phosphoglucomutase activity by 50 % , a bimodal distribution among the population tested was obtained .
	manualset3
204008	1	417609	7	NULL	NULL	0	NULL	women ( Study 1 )	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When women ( Study 1 ) , African Americans ( Study 2 ) , and Americans ( Study 3 ) simply thought about suspected prejudice against their ingroup , categorization guided their perceptions : Participants assimilated their views of the prejudiced event toward the perceptions of ingroup members but contrasted away from the perceptions of outgroup members .
	manualset3
204009	2	417609	7	NULL	NULL	0	NULL	African Americans ( Study 2 )	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When women ( Study 1 ) , African Americans ( Study 2 ) , and Americans ( Study 3 ) simply thought about suspected prejudice against their ingroup , categorization guided their perceptions : Participants assimilated their views of the prejudiced event toward the perceptions of ingroup members but contrasted away from the perceptions of outgroup members .
	manualset3
204010	3	417609	7	NULL	NULL	0	NULL	Americans ( Study 3 )	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When women ( Study 1 ) , African Americans ( Study 2 ) , and Americans ( Study 3 ) simply thought about suspected prejudice against their ingroup , categorization guided their perceptions : Participants assimilated their views of the prejudiced event toward the perceptions of ingroup members but contrasted away from the perceptions of outgroup members .
	manualset3
204011	4	417609	7	NULL	NULL	0	NULL	ingroup	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When women ( Study 1 ) , African Americans ( Study 2 ) , and Americans ( Study 3 ) simply thought about suspected prejudice against their ingroup , categorization guided their perceptions : Participants assimilated their views of the prejudiced event toward the perceptions of ingroup members but contrasted away from the perceptions of outgroup members .
	manualset3
204012	5	417609	7	NULL	NULL	0	NULL	categorization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When women ( Study 1 ) , African Americans ( Study 2 ) , and Americans ( Study 3 ) simply thought about suspected prejudice against their ingroup , categorization guided their perceptions : Participants assimilated their views of the prejudiced event toward the perceptions of ingroup members but contrasted away from the perceptions of outgroup members .
	manualset3
204013	6	417609	7	NULL	NULL	0	NULL	perceptions	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When women ( Study 1 ) , African Americans ( Study 2 ) , and Americans ( Study 3 ) simply thought about suspected prejudice against their ingroup , categorization guided their perceptions : Participants assimilated their views of the prejudiced event toward the perceptions of ingroup members but contrasted away from the perceptions of outgroup members .
	manualset3
204014	7	417609	7	NULL	NULL	0	NULL	Participants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When women ( Study 1 ) , African Americans ( Study 2 ) , and Americans ( Study 3 ) simply thought about suspected prejudice against their ingroup , categorization guided their perceptions : Participants assimilated their views of the prejudiced event toward the perceptions of ingroup members but contrasted away from the perceptions of outgroup members .
	manualset3
204015	8	417609	7	NULL	NULL	0	NULL	views 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When women ( Study 1 ) , African Americans ( Study 2 ) , and Americans ( Study 3 ) simply thought about suspected prejudice against their ingroup , categorization guided their perceptions : Participants assimilated their views of the prejudiced event toward the perceptions of ingroup members but contrasted away from the perceptions of outgroup members .
	manualset3
204016	9	417609	7	NULL	NULL	0	NULL	prejudiced event	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When women ( Study 1 ) , African Americans ( Study 2 ) , and Americans ( Study 3 ) simply thought about suspected prejudice against their ingroup , categorization guided their perceptions : Participants assimilated their views of the prejudiced event toward the perceptions of ingroup members but contrasted away from the perceptions of outgroup members .
	manualset3
204017	10	417609	7	NULL	NULL	0	NULL	perceptions	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When women ( Study 1 ) , African Americans ( Study 2 ) , and Americans ( Study 3 ) simply thought about suspected prejudice against their ingroup , categorization guided their perceptions : Participants assimilated their views of the prejudiced event toward the perceptions of ingroup members but contrasted away from the perceptions of outgroup members .
	manualset3
204018	11	417609	7	NULL	NULL	0	NULL	ingroup members	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When women ( Study 1 ) , African Americans ( Study 2 ) , and Americans ( Study 3 ) simply thought about suspected prejudice against their ingroup , categorization guided their perceptions : Participants assimilated their views of the prejudiced event toward the perceptions of ingroup members but contrasted away from the perceptions of outgroup members .
	manualset3
204019	13	417609	7	NULL	NULL	NULL	NULL	outgroup members	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When women ( Study 1 ) , African Americans ( Study 2 ) , and Americans ( Study 3 ) simply thought about suspected prejudice against their ingroup , categorization guided their perceptions : Participants assimilated their views of the prejudiced event toward the perceptions of ingroup members but contrasted away from the perceptions of outgroup members .
	manualset3
204020	12	417609	7	NULL	NULL	0	NULL	perceptions	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When women ( Study 1 ) , African Americans ( Study 2 ) , and Americans ( Study 3 ) simply thought about suspected prejudice against their ingroup , categorization guided their perceptions : Participants assimilated their views of the prejudiced event toward the perceptions of ingroup members but contrasted away from the perceptions of outgroup members .
	manualset3
204021	1	417610	7	NULL	NULL	0	NULL	POD	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Where POD was the principle outcome , studies must have employed the DSM or ICD criteria .
	manualset3
204022	2	417610	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Where POD was the principle outcome , studies must have employed the DSM or ICD criteria .
	manualset3
204023	3	417610	7	NULL	NULL	0	NULL	DSM criteria	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Where POD was the principle outcome , studies must have employed the DSM or ICD criteria .
	manualset3
204024	4	417610	7	NULL	NULL	0	NULL	ICD criteria	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Where POD was the principle outcome , studies must have employed the DSM or ICD criteria .
	manualset3
204025	1	417611	7	NULL	NULL	0	NULL	 Cost-effectiveness analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cost-effectiveness analysis of nuclear cardiology and its impact on total expense for diagnosis of coronary artery disease ) .
	manualset3
204026	2	417611	7	NULL	NULL	0	NULL	 nuclear cardiology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cost-effectiveness analysis of nuclear cardiology and its impact on total expense for diagnosis of coronary artery disease ) .
	manualset3
204027	3	417611	7	NULL	NULL	0	NULL	impact	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cost-effectiveness analysis of nuclear cardiology and its impact on total expense for diagnosis of coronary artery disease ) .
	manualset3
204028	4	417611	7	NULL	NULL	0	NULL	total expense	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cost-effectiveness analysis of nuclear cardiology and its impact on total expense for diagnosis of coronary artery disease ) .
	manualset3
204029	5	417611	7	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cost-effectiveness analysis of nuclear cardiology and its impact on total expense for diagnosis of coronary artery disease ) .
	manualset3
204030	6	417611	7	NULL	NULL	0	NULL	coronary artery disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cost-effectiveness analysis of nuclear cardiology and its impact on total expense for diagnosis of coronary artery disease ) .
	manualset3
204031	1	417612	7	NULL	NULL	0	NULL	pre-conception guidelines	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Where available , pre-conception guidelines for men using these medications for RA are also discussed .
	manualset3
204032	2	417612	7	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Where available , pre-conception guidelines for men using these medications for RA are also discussed .
	manualset3
204033	3	417612	7	NULL	NULL	0	NULL	medications	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Where available , pre-conception guidelines for men using these medications for RA are also discussed .
	manualset3
204034	4	417612	7	NULL	NULL	0	NULL	RA	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Where available , pre-conception guidelines for men using these medications for RA are also discussed .
	manualset3
204040	1	417613	7	NULL	NULL	0	NULL	information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Where can I find information regarding the potassium and phosphorus content of foods ?
	manualset3
204041	2	417613	7	NULL	NULL	0	NULL	potassium content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Where can I find information regarding the potassium and phosphorus content of foods ?
	manualset3
204042	3	417613	7	NULL	NULL	0	NULL	phosphorus content 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Where can I find information regarding the potassium and phosphorus content of foods ?
	manualset3
204043	4	417613	7	NULL	NULL	0	NULL	 foods	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Where can I find information regarding the potassium and phosphorus content of foods ?
	manualset3
204066	1	417614	7	NULL	NULL	NULL	NULL	 amplitude reduction	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Where obvious amplitude reduction occurred with maturation and aging among nonretarded subjects , amplitude changes were generally absent among Down 's syndrome subjects .
	manualset3
204069	2	417614	7	NULL	NULL	0	NULL	maturation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Where obvious amplitude reduction occurred with maturation and aging among nonretarded subjects , amplitude changes were generally absent among Down 's syndrome subjects .
	manualset3
204070	3	417614	7	NULL	NULL	0	NULL	aging	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Where obvious amplitude reduction occurred with maturation and aging among nonretarded subjects , amplitude changes were generally absent among Down 's syndrome subjects .
	manualset3
204071	4	417614	7	NULL	NULL	0	NULL	 nonretarded subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Where obvious amplitude reduction occurred with maturation and aging among nonretarded subjects , amplitude changes were generally absent among Down 's syndrome subjects .
	manualset3
204072	5	417614	7	NULL	NULL	0	NULL	amplitude changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Where obvious amplitude reduction occurred with maturation and aging among nonretarded subjects , amplitude changes were generally absent among Down 's syndrome subjects .
	manualset3
204073	6	417614	7	NULL	NULL	0	NULL	Down 's syndrome subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Where obvious amplitude reduction occurred with maturation and aging among nonretarded subjects , amplitude changes were generally absent among Down 's syndrome subjects .
	manualset3
204097	1	417615	7	NULL	NULL	0	NULL	AMPK knockdown	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas AMPK knockdown prevented the enhanced basal and insulin-stimulated GLUT4myc labeling by AICAR and DNP , cholesterol replenishment only blocked the AMPK-associated enhancement in insulin action .
	manualset3
204099	2	417615	7	NULL	NULL	0	NULL	enhanced basal GLUT4myc labeling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas AMPK knockdown prevented the enhanced basal and insulin-stimulated GLUT4myc labeling by AICAR and DNP , cholesterol replenishment only blocked the AMPK-associated enhancement in insulin action .
	manualset3
204100	3	417615	7	NULL	NULL	0	NULL	insulin-stimulated GLUT4myc labeling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas AMPK knockdown prevented the enhanced basal and insulin-stimulated GLUT4myc labeling by AICAR and DNP , cholesterol replenishment only blocked the AMPK-associated enhancement in insulin action .
	manualset3
204104	4	417615	7	NULL	NULL	0	NULL	AICAR	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas AMPK knockdown prevented the enhanced basal and insulin-stimulated GLUT4myc labeling by AICAR and DNP , cholesterol replenishment only blocked the AMPK-associated enhancement in insulin action .
	manualset3
204105	5	417615	7	NULL	NULL	0	NULL	DNP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas AMPK knockdown prevented the enhanced basal and insulin-stimulated GLUT4myc labeling by AICAR and DNP , cholesterol replenishment only blocked the AMPK-associated enhancement in insulin action .
	manualset3
204106	6	417615	7	NULL	NULL	0	NULL	cholesterol replenishment	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas AMPK knockdown prevented the enhanced basal and insulin-stimulated GLUT4myc labeling by AICAR and DNP , cholesterol replenishment only blocked the AMPK-associated enhancement in insulin action .
	manualset3
204107	7	417615	7	NULL	NULL	0	NULL	AMPK-associated enhancement	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas AMPK knockdown prevented the enhanced basal and insulin-stimulated GLUT4myc labeling by AICAR and DNP , cholesterol replenishment only blocked the AMPK-associated enhancement in insulin action .
	manualset3
204108	8	417615	7	NULL	NULL	0	NULL	insulin action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas AMPK knockdown prevented the enhanced basal and insulin-stimulated GLUT4myc labeling by AICAR and DNP , cholesterol replenishment only blocked the AMPK-associated enhancement in insulin action .
	manualset3
204109	1	417616	7	NULL	NULL	0	NULL	voxel size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas a voxel size in our images is mere 1/1 , 200 compared to that reported about the prototype human NMR imaging devices , high resolution has been realized .
	manualset3
204110	2	417616	7	NULL	NULL	0	NULL	 images	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas a voxel size in our images is mere 1/1 , 200 compared to that reported about the prototype human NMR imaging devices , high resolution has been realized .
	manualset3
204112	3	417616	7	NULL	NULL	0	NULL	 1/1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas a voxel size in our images is mere 1/1 , 200 compared to that reported about the prototype human NMR imaging devices , high resolution has been realized .
	manualset3
204116	4	417616	7	NULL	NULL	0	NULL	200 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas a voxel size in our images is mere 1/1 , 200 compared to that reported about the prototype human NMR imaging devices , high resolution has been realized .
	manualset3
204117	5	417616	7	NULL	NULL	0	NULL	prototype human NMR imaging devices	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas a voxel size in our images is mere 1/1 , 200 compared to that reported about the prototype human NMR imaging devices , high resolution has been realized .
	manualset3
204118	6	417616	7	NULL	NULL	0	NULL	high resolution	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas a voxel size in our images is mere 1/1 , 200 compared to that reported about the prototype human NMR imaging devices , high resolution has been realized .
	manualset3
204120	1	417617	7	NULL	NULL	0	NULL	control myoblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas control myoblasts fuse to form branched myotubes with aligned nuclei , FSHD myoblasts fuse to form either thin and branched myotubes with aligned nuclei or large myotubes with random nuclei distribution .
	manualset3
204122	2	417617	7	NULL	NULL	0	NULL	branched myotubes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas control myoblasts fuse to form branched myotubes with aligned nuclei , FSHD myoblasts fuse to form either thin and branched myotubes with aligned nuclei or large myotubes with random nuclei distribution .
	manualset3
204124	3	417617	7	NULL	NULL	0	NULL	nuclei	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas control myoblasts fuse to form branched myotubes with aligned nuclei , FSHD myoblasts fuse to form either thin and branched myotubes with aligned nuclei or large myotubes with random nuclei distribution .
	manualset3
204126	4	417617	7	NULL	NULL	0	NULL	FSHD myoblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas control myoblasts fuse to form branched myotubes with aligned nuclei , FSHD myoblasts fuse to form either thin and branched myotubes with aligned nuclei or large myotubes with random nuclei distribution .
	manualset3
204128	5	417617	7	NULL	NULL	0	NULL	thin myotubes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas control myoblasts fuse to form branched myotubes with aligned nuclei , FSHD myoblasts fuse to form either thin and branched myotubes with aligned nuclei or large myotubes with random nuclei distribution .
	manualset3
204129	6	417617	7	NULL	NULL	0	NULL	 branched myotubes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas control myoblasts fuse to form branched myotubes with aligned nuclei , FSHD myoblasts fuse to form either thin and branched myotubes with aligned nuclei or large myotubes with random nuclei distribution .
	manualset3
204130	7	417617	7	NULL	NULL	0	NULL	 aligned nuclei	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas control myoblasts fuse to form branched myotubes with aligned nuclei , FSHD myoblasts fuse to form either thin and branched myotubes with aligned nuclei or large myotubes with random nuclei distribution .
	manualset3
204131	8	417617	7	NULL	NULL	0	NULL	large myotubes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas control myoblasts fuse to form branched myotubes with aligned nuclei , FSHD myoblasts fuse to form either thin and branched myotubes with aligned nuclei or large myotubes with random nuclei distribution .
	manualset3
204132	9	417617	7	NULL	NULL	0	NULL	random nuclei distribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas control myoblasts fuse to form branched myotubes with aligned nuclei , FSHD myoblasts fuse to form either thin and branched myotubes with aligned nuclei or large myotubes with random nuclei distribution .
	manualset3
204133	1	417618	7	NULL	NULL	0	NULL	 hippocampus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas it is widely agreed that the hippocampus supports recollection ( remembering the episode in which an item was learned ) , there is uncertainty about whether it also supports familiarity ( simply knowing that an item was encountered but without remembering the learning episode ) .
	manualset3
204137	2	417618	7	NULL	NULL	0	NULL	recollection	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas it is widely agreed that the hippocampus supports recollection ( remembering the episode in which an item was learned ) , there is uncertainty about whether it also supports familiarity ( simply knowing that an item was encountered but without remembering the learning episode ) .
	manualset3
204138	3	417618	7	NULL	NULL	0	NULL	episode	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas it is widely agreed that the hippocampus supports recollection ( remembering the episode in which an item was learned ) , there is uncertainty about whether it also supports familiarity ( simply knowing that an item was encountered but without remembering the learning episode ) .
	manualset3
204142	4	417618	7	NULL	NULL	0	NULL	familiarity	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas it is widely agreed that the hippocampus supports recollection ( remembering the episode in which an item was learned ) , there is uncertainty about whether it also supports familiarity ( simply knowing that an item was encountered but without remembering the learning episode ) .
	manualset3
204151	6	417618	7	NULL	NULL	NULL	NULL	learning episode	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Whereas it is widely agreed that the hippocampus supports recollection ( remembering the episode in which an item was learned ) , there is uncertainty about whether it also supports familiarity ( simply knowing that an item was encountered but without remembering the learning episode ) .
	manualset3
204153	5	417618	7	NULL	NULL	0	NULL	item	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas it is widely agreed that the hippocampus supports recollection ( remembering the episode in which an item was learned ) , there is uncertainty about whether it also supports familiarity ( simply knowing that an item was encountered but without remembering the learning episode ) .
	manualset3
204154	7	417618	7	NULL	NULL	0	NULL	item	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas it is widely agreed that the hippocampus supports recollection ( remembering the episode in which an item was learned ) , there is uncertainty about whether it also supports familiarity ( simply knowing that an item was encountered but without remembering the learning episode ) .
	manualset3
204155	1	417619	7	NULL	NULL	0	NULL	understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas our understanding of its pathophysiology is limited , postmortem studies suggest that schizophrenia is associated with deficits of GABA-mediated synaptic transmission .
	manualset3
204156	2	417619	7	NULL	NULL	0	NULL	pathophysiology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas our understanding of its pathophysiology is limited , postmortem studies suggest that schizophrenia is associated with deficits of GABA-mediated synaptic transmission .
	manualset3
204157	3	417619	7	NULL	NULL	0	NULL	postmortem studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas our understanding of its pathophysiology is limited , postmortem studies suggest that schizophrenia is associated with deficits of GABA-mediated synaptic transmission .
	manualset3
204158	4	417619	7	NULL	NULL	0	NULL	schizophrenia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas our understanding of its pathophysiology is limited , postmortem studies suggest that schizophrenia is associated with deficits of GABA-mediated synaptic transmission .
	manualset3
204159	5	417619	7	NULL	NULL	0	NULL	deficits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas our understanding of its pathophysiology is limited , postmortem studies suggest that schizophrenia is associated with deficits of GABA-mediated synaptic transmission .
	manualset3
204160	6	417619	7	NULL	NULL	0	NULL	GABA-mediated synaptic transmission	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas our understanding of its pathophysiology is limited , postmortem studies suggest that schizophrenia is associated with deficits of GABA-mediated synaptic transmission .
	manualset3
204161	1	417620	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients exhibited typical clinical features of LHON .
	manualset3
204162	2	417620	7	NULL	NULL	0	NULL	clinical features	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients exhibited typical clinical features of LHON .
	manualset3
204163	3	417620	7	NULL	NULL	0	NULL	LHON 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients exhibited typical clinical features of LHON .
	manualset3
204164	1	417621	7	NULL	NULL	0	NULL	 taurine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas taurine inhibited the luminol chemiluminescence of an H2O2/HOC1 system by HOC1 scavenging , this compound had little effect on myeloperoxidase/H2O2-dependent luminol chemiluminescence ; in contrast , 10 microM-salicylhydroxamic acid did not quench HOC1 significantly but greatly diminished myeloperoxidase/H2O2-dependent luminol chemiluminescence , indicating that its effects on myeloperoxidase chemiluminescence were largely due to peroxidase inhibition rather than non-specific HOC1 scavenging .
	manualset3
204165	2	417621	7	NULL	NULL	NULL	NULL	luminol chemiluminescence	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Whereas taurine inhibited the luminol chemiluminescence of an H2O2/HOC1 system by HOC1 scavenging , this compound had little effect on myeloperoxidase/H2O2-dependent luminol chemiluminescence ; in contrast , 10 microM-salicylhydroxamic acid did not quench HOC1 significantly but greatly diminished myeloperoxidase/H2O2-dependent luminol chemiluminescence , indicating that its effects on myeloperoxidase chemiluminescence were largely due to peroxidase inhibition rather than non-specific HOC1 scavenging .
	manualset3
204166	3	417621	7	NULL	NULL	0	NULL	H2O2/HOC1 system	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas taurine inhibited the luminol chemiluminescence of an H2O2/HOC1 system by HOC1 scavenging , this compound had little effect on myeloperoxidase/H2O2-dependent luminol chemiluminescence ; in contrast , 10 microM-salicylhydroxamic acid did not quench HOC1 significantly but greatly diminished myeloperoxidase/H2O2-dependent luminol chemiluminescence , indicating that its effects on myeloperoxidase chemiluminescence were largely due to peroxidase inhibition rather than non-specific HOC1 scavenging .
	manualset3
204167	4	417621	7	NULL	NULL	NULL	NULL	HOC1 scavenging	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Whereas taurine inhibited the luminol chemiluminescence of an H2O2/HOC1 system by HOC1 scavenging , this compound had little effect on myeloperoxidase/H2O2-dependent luminol chemiluminescence ; in contrast , 10 microM-salicylhydroxamic acid did not quench HOC1 significantly but greatly diminished myeloperoxidase/H2O2-dependent luminol chemiluminescence , indicating that its effects on myeloperoxidase chemiluminescence were largely due to peroxidase inhibition rather than non-specific HOC1 scavenging .
	manualset3
204168	5	417621	7	NULL	NULL	0	NULL	compound 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas taurine inhibited the luminol chemiluminescence of an H2O2/HOC1 system by HOC1 scavenging , this compound had little effect on myeloperoxidase/H2O2-dependent luminol chemiluminescence ; in contrast , 10 microM-salicylhydroxamic acid did not quench HOC1 significantly but greatly diminished myeloperoxidase/H2O2-dependent luminol chemiluminescence , indicating that its effects on myeloperoxidase chemiluminescence were largely due to peroxidase inhibition rather than non-specific HOC1 scavenging .
	manualset3
204169	6	417621	7	NULL	NULL	NULL	NULL	myeloperoxidase/H2O2-dependent luminol chemiluminescence	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Whereas taurine inhibited the luminol chemiluminescence of an H2O2/HOC1 system by HOC1 scavenging , this compound had little effect on myeloperoxidase/H2O2-dependent luminol chemiluminescence ; in contrast , 10 microM-salicylhydroxamic acid did not quench HOC1 significantly but greatly diminished myeloperoxidase/H2O2-dependent luminol chemiluminescence , indicating that its effects on myeloperoxidase chemiluminescence were largely due to peroxidase inhibition rather than non-specific HOC1 scavenging .
	manualset3
204170	7	417621	7	NULL	NULL	0	NULL	10 microM-salicylhydroxamic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas taurine inhibited the luminol chemiluminescence of an H2O2/HOC1 system by HOC1 scavenging , this compound had little effect on myeloperoxidase/H2O2-dependent luminol chemiluminescence ; in contrast , 10 microM-salicylhydroxamic acid did not quench HOC1 significantly but greatly diminished myeloperoxidase/H2O2-dependent luminol chemiluminescence , indicating that its effects on myeloperoxidase chemiluminescence were largely due to peroxidase inhibition rather than non-specific HOC1 scavenging .
	manualset3
204171	8	417621	7	NULL	NULL	0	NULL	HOC1	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas taurine inhibited the luminol chemiluminescence of an H2O2/HOC1 system by HOC1 scavenging , this compound had little effect on myeloperoxidase/H2O2-dependent luminol chemiluminescence ; in contrast , 10 microM-salicylhydroxamic acid did not quench HOC1 significantly but greatly diminished myeloperoxidase/H2O2-dependent luminol chemiluminescence , indicating that its effects on myeloperoxidase chemiluminescence were largely due to peroxidase inhibition rather than non-specific HOC1 scavenging .
	manualset3
204172	9	417621	7	NULL	NULL	NULL	NULL	myeloperoxidase/H2O2-dependent luminol chemiluminescence	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Whereas taurine inhibited the luminol chemiluminescence of an H2O2/HOC1 system by HOC1 scavenging , this compound had little effect on myeloperoxidase/H2O2-dependent luminol chemiluminescence ; in contrast , 10 microM-salicylhydroxamic acid did not quench HOC1 significantly but greatly diminished myeloperoxidase/H2O2-dependent luminol chemiluminescence , indicating that its effects on myeloperoxidase chemiluminescence were largely due to peroxidase inhibition rather than non-specific HOC1 scavenging .
	manualset3
204173	10	417621	7	NULL	NULL	0	NULL	myeloperoxidase chemiluminescence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas taurine inhibited the luminol chemiluminescence of an H2O2/HOC1 system by HOC1 scavenging , this compound had little effect on myeloperoxidase/H2O2-dependent luminol chemiluminescence ; in contrast , 10 microM-salicylhydroxamic acid did not quench HOC1 significantly but greatly diminished myeloperoxidase/H2O2-dependent luminol chemiluminescence , indicating that its effects on myeloperoxidase chemiluminescence were largely due to peroxidase inhibition rather than non-specific HOC1 scavenging .
	manualset3
204174	11	417621	7	NULL	NULL	0	NULL	peroxidase inhibition 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas taurine inhibited the luminol chemiluminescence of an H2O2/HOC1 system by HOC1 scavenging , this compound had little effect on myeloperoxidase/H2O2-dependent luminol chemiluminescence ; in contrast , 10 microM-salicylhydroxamic acid did not quench HOC1 significantly but greatly diminished myeloperoxidase/H2O2-dependent luminol chemiluminescence , indicating that its effects on myeloperoxidase chemiluminescence were largely due to peroxidase inhibition rather than non-specific HOC1 scavenging .
	manualset3
204175	12	417621	7	NULL	NULL	0	NULL	non-specific HOC1 scavenging 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas taurine inhibited the luminol chemiluminescence of an H2O2/HOC1 system by HOC1 scavenging , this compound had little effect on myeloperoxidase/H2O2-dependent luminol chemiluminescence ; in contrast , 10 microM-salicylhydroxamic acid did not quench HOC1 significantly but greatly diminished myeloperoxidase/H2O2-dependent luminol chemiluminescence , indicating that its effects on myeloperoxidase chemiluminescence were largely due to peroxidase inhibition rather than non-specific HOC1 scavenging .
	manualset3
204176	1	417622	7	NULL	NULL	0	NULL	C-terminal domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas the C-terminal domain of Hc1 between amino acids 63 and 125 shows best alignment with sea-urchin histone H1 , and N-terminus between amino acids 1 and 62 is highly conserved among various chlamydial species , suggesting a bifunctional role for this unique protein .
	manualset3
204177	2	417622	7	NULL	NULL	0	NULL	Hc1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas the C-terminal domain of Hc1 between amino acids 63 and 125 shows best alignment with sea-urchin histone H1 , and N-terminus between amino acids 1 and 62 is highly conserved among various chlamydial species , suggesting a bifunctional role for this unique protein .
	manualset3
204178	3	417622	7	NULL	NULL	NULL	NULL	amino acids 63	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Whereas the C-terminal domain of Hc1 between amino acids 63 and 125 shows best alignment with sea-urchin histone H1 , and N-terminus between amino acids 1 and 62 is highly conserved among various chlamydial species , suggesting a bifunctional role for this unique protein .
	manualset3
204179	4	417622	7	NULL	NULL	0	NULL	amino acids 125	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas the C-terminal domain of Hc1 between amino acids 63 and 125 shows best alignment with sea-urchin histone H1 , and N-terminus between amino acids 1 and 62 is highly conserved among various chlamydial species , suggesting a bifunctional role for this unique protein .
	manualset3
204180	5	417622	7	NULL	NULL	0	NULL	best alignment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas the C-terminal domain of Hc1 between amino acids 63 and 125 shows best alignment with sea-urchin histone H1 , and N-terminus between amino acids 1 and 62 is highly conserved among various chlamydial species , suggesting a bifunctional role for this unique protein .
	manualset3
204181	6	417622	7	NULL	NULL	0	NULL	sea-urchin histone H1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas the C-terminal domain of Hc1 between amino acids 63 and 125 shows best alignment with sea-urchin histone H1 , and N-terminus between amino acids 1 and 62 is highly conserved among various chlamydial species , suggesting a bifunctional role for this unique protein .
	manualset3
204182	7	417622	7	NULL	NULL	0	NULL	N-terminus	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas the C-terminal domain of Hc1 between amino acids 63 and 125 shows best alignment with sea-urchin histone H1 , and N-terminus between amino acids 1 and 62 is highly conserved among various chlamydial species , suggesting a bifunctional role for this unique protein .
	manualset3
204183	8	417622	7	NULL	NULL	0	NULL	amino acids 1	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas the C-terminal domain of Hc1 between amino acids 63 and 125 shows best alignment with sea-urchin histone H1 , and N-terminus between amino acids 1 and 62 is highly conserved among various chlamydial species , suggesting a bifunctional role for this unique protein .
	manualset3
204184	9	417622	7	NULL	NULL	0	NULL	amino acids 62	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas the C-terminal domain of Hc1 between amino acids 63 and 125 shows best alignment with sea-urchin histone H1 , and N-terminus between amino acids 1 and 62 is highly conserved among various chlamydial species , suggesting a bifunctional role for this unique protein .
	manualset3
204185	10	417622	7	NULL	NULL	0	NULL	chlamydial species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas the C-terminal domain of Hc1 between amino acids 63 and 125 shows best alignment with sea-urchin histone H1 , and N-terminus between amino acids 1 and 62 is highly conserved among various chlamydial species , suggesting a bifunctional role for this unique protein .
	manualset3
204186	11	417622	7	NULL	NULL	0	NULL	bifunctional role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas the C-terminal domain of Hc1 between amino acids 63 and 125 shows best alignment with sea-urchin histone H1 , and N-terminus between amino acids 1 and 62 is highly conserved among various chlamydial species , suggesting a bifunctional role for this unique protein .
	manualset3
204187	12	417622	7	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas the C-terminal domain of Hc1 between amino acids 63 and 125 shows best alignment with sea-urchin histone H1 , and N-terminus between amino acids 1 and 62 is highly conserved among various chlamydial species , suggesting a bifunctional role for this unique protein .
	manualset3
204188	1	417623	7	NULL	NULL	0	NULL	 effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas these effects may be largely beneficial , dose-related side effects could have implications for the safe therapeutic use of rHuEPO and its illegal use as a performance-enhancing agent in endurance sports .
	manualset3
204189	2	417623	7	NULL	NULL	0	NULL	dose-related side effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas these effects may be largely beneficial , dose-related side effects could have implications for the safe therapeutic use of rHuEPO and its illegal use as a performance-enhancing agent in endurance sports .
	manualset3
204190	3	417623	7	NULL	NULL	0	NULL	implications 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas these effects may be largely beneficial , dose-related side effects could have implications for the safe therapeutic use of rHuEPO and its illegal use as a performance-enhancing agent in endurance sports .
	manualset3
204191	4	417623	7	NULL	NULL	0	NULL	therapeutic use	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas these effects may be largely beneficial , dose-related side effects could have implications for the safe therapeutic use of rHuEPO and its illegal use as a performance-enhancing agent in endurance sports .
	manualset3
204192	5	417623	7	NULL	NULL	0	NULL	 rHuEPO	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas these effects may be largely beneficial , dose-related side effects could have implications for the safe therapeutic use of rHuEPO and its illegal use as a performance-enhancing agent in endurance sports .
	manualset3
204195	6	417623	7	NULL	NULL	0	NULL	performance-enhancing agent	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas these effects may be largely beneficial , dose-related side effects could have implications for the safe therapeutic use of rHuEPO and its illegal use as a performance-enhancing agent in endurance sports .
	manualset3
204196	7	417623	7	NULL	NULL	0	NULL	endurance sports	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas these effects may be largely beneficial , dose-related side effects could have implications for the safe therapeutic use of rHuEPO and its illegal use as a performance-enhancing agent in endurance sports .
	manualset3
204197	1	417624	7	NULL	NULL	0	NULL	transduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas transduction of marker genes ( LacZ or enhanced green fluorescence protein ( EGFP ) ) did not alter their potent allostimulatory activity , DC transduced with CTLA4lg exhibited striking reductions in cell surface staining for CD86 , but not MHC class II , and were poor stimulators of T cell proliferation and cytotoxic T lymphocyte ( CTL ) responses .
	manualset3
204198	2	417624	7	NULL	NULL	0	NULL	marker genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas transduction of marker genes ( LacZ or enhanced green fluorescence protein ( EGFP ) ) did not alter their potent allostimulatory activity , DC transduced with CTLA4lg exhibited striking reductions in cell surface staining for CD86 , but not MHC class II , and were poor stimulators of T cell proliferation and cytotoxic T lymphocyte ( CTL ) responses .
	manualset3
204199	3	417624	7	NULL	NULL	0	NULL	LacZ	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas transduction of marker genes ( LacZ or enhanced green fluorescence protein ( EGFP ) ) did not alter their potent allostimulatory activity , DC transduced with CTLA4lg exhibited striking reductions in cell surface staining for CD86 , but not MHC class II , and were poor stimulators of T cell proliferation and cytotoxic T lymphocyte ( CTL ) responses .
	manualset3
204200	4	417624	7	NULL	NULL	0	NULL	enhanced green fluorescence protein ( EGFP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas transduction of marker genes ( LacZ or enhanced green fluorescence protein ( EGFP ) ) did not alter their potent allostimulatory activity , DC transduced with CTLA4lg exhibited striking reductions in cell surface staining for CD86 , but not MHC class II , and were poor stimulators of T cell proliferation and cytotoxic T lymphocyte ( CTL ) responses .
	manualset3
204201	5	417624	7	NULL	NULL	0	NULL	 allostimulatory activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas transduction of marker genes ( LacZ or enhanced green fluorescence protein ( EGFP ) ) did not alter their potent allostimulatory activity , DC transduced with CTLA4lg exhibited striking reductions in cell surface staining for CD86 , but not MHC class II , and were poor stimulators of T cell proliferation and cytotoxic T lymphocyte ( CTL ) responses .
	manualset3
204202	6	417624	7	NULL	NULL	0	NULL	DC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas transduction of marker genes ( LacZ or enhanced green fluorescence protein ( EGFP ) ) did not alter their potent allostimulatory activity , DC transduced with CTLA4lg exhibited striking reductions in cell surface staining for CD86 , but not MHC class II , and were poor stimulators of T cell proliferation and cytotoxic T lymphocyte ( CTL ) responses .
	manualset3
204203	7	417624	7	NULL	NULL	0	NULL	 CTLA4lg	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas transduction of marker genes ( LacZ or enhanced green fluorescence protein ( EGFP ) ) did not alter their potent allostimulatory activity , DC transduced with CTLA4lg exhibited striking reductions in cell surface staining for CD86 , but not MHC class II , and were poor stimulators of T cell proliferation and cytotoxic T lymphocyte ( CTL ) responses .
	manualset3
204205	8	417624	7	NULL	NULL	0	NULL	reductions	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas transduction of marker genes ( LacZ or enhanced green fluorescence protein ( EGFP ) ) did not alter their potent allostimulatory activity , DC transduced with CTLA4lg exhibited striking reductions in cell surface staining for CD86 , but not MHC class II , and were poor stimulators of T cell proliferation and cytotoxic T lymphocyte ( CTL ) responses .
	manualset3
204206	9	417624	7	NULL	NULL	0	NULL	cell surface staining	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas transduction of marker genes ( LacZ or enhanced green fluorescence protein ( EGFP ) ) did not alter their potent allostimulatory activity , DC transduced with CTLA4lg exhibited striking reductions in cell surface staining for CD86 , but not MHC class II , and were poor stimulators of T cell proliferation and cytotoxic T lymphocyte ( CTL ) responses .
	manualset3
204207	10	417624	7	NULL	NULL	0	NULL	CD86	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas transduction of marker genes ( LacZ or enhanced green fluorescence protein ( EGFP ) ) did not alter their potent allostimulatory activity , DC transduced with CTLA4lg exhibited striking reductions in cell surface staining for CD86 , but not MHC class II , and were poor stimulators of T cell proliferation and cytotoxic T lymphocyte ( CTL ) responses .
	manualset3
204208	11	417624	7	NULL	NULL	0	NULL	MHC class II	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas transduction of marker genes ( LacZ or enhanced green fluorescence protein ( EGFP ) ) did not alter their potent allostimulatory activity , DC transduced with CTLA4lg exhibited striking reductions in cell surface staining for CD86 , but not MHC class II , and were poor stimulators of T cell proliferation and cytotoxic T lymphocyte ( CTL ) responses .
	manualset3
204209	12	417624	7	NULL	NULL	0	NULL	stimulators	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas transduction of marker genes ( LacZ or enhanced green fluorescence protein ( EGFP ) ) did not alter their potent allostimulatory activity , DC transduced with CTLA4lg exhibited striking reductions in cell surface staining for CD86 , but not MHC class II , and were poor stimulators of T cell proliferation and cytotoxic T lymphocyte ( CTL ) responses .
	manualset3
204210	13	417624	7	NULL	NULL	0	NULL	T cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas transduction of marker genes ( LacZ or enhanced green fluorescence protein ( EGFP ) ) did not alter their potent allostimulatory activity , DC transduced with CTLA4lg exhibited striking reductions in cell surface staining for CD86 , but not MHC class II , and were poor stimulators of T cell proliferation and cytotoxic T lymphocyte ( CTL ) responses .
	manualset3
204212	14	417624	7	NULL	NULL	0	NULL	cytotoxic T lymphocyte ( CTL ) responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas transduction of marker genes ( LacZ or enhanced green fluorescence protein ( EGFP ) ) did not alter their potent allostimulatory activity , DC transduced with CTLA4lg exhibited striking reductions in cell surface staining for CD86 , but not MHC class II , and were poor stimulators of T cell proliferation and cytotoxic T lymphocyte ( CTL ) responses .
	manualset3
204218	1	417625	7	NULL	NULL	0	NULL	unsolvated lithiated arginine	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas unsolvated lithiated arginine is nonzwitterionic , these results provide compelling evidence that attachment of a single water molecule to this ion makes the zwitterionic form of arginine , in which the side chain is protonated , more stable .
	manualset3
204220	2	417625	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas unsolvated lithiated arginine is nonzwitterionic , these results provide compelling evidence that attachment of a single water molecule to this ion makes the zwitterionic form of arginine , in which the side chain is protonated , more stable .
	manualset3
204222	3	417625	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas unsolvated lithiated arginine is nonzwitterionic , these results provide compelling evidence that attachment of a single water molecule to this ion makes the zwitterionic form of arginine , in which the side chain is protonated , more stable .
	manualset3
204223	4	417625	7	NULL	NULL	0	NULL	attachment 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas unsolvated lithiated arginine is nonzwitterionic , these results provide compelling evidence that attachment of a single water molecule to this ion makes the zwitterionic form of arginine , in which the side chain is protonated , more stable .
	manualset3
204224	5	417625	7	NULL	NULL	0	NULL	single water molecule	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas unsolvated lithiated arginine is nonzwitterionic , these results provide compelling evidence that attachment of a single water molecule to this ion makes the zwitterionic form of arginine , in which the side chain is protonated , more stable .
	manualset3
204225	6	417625	7	NULL	NULL	0	NULL	ion	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas unsolvated lithiated arginine is nonzwitterionic , these results provide compelling evidence that attachment of a single water molecule to this ion makes the zwitterionic form of arginine , in which the side chain is protonated , more stable .
	manualset3
204226	7	417625	7	NULL	NULL	0	NULL	zwitterionic form	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas unsolvated lithiated arginine is nonzwitterionic , these results provide compelling evidence that attachment of a single water molecule to this ion makes the zwitterionic form of arginine , in which the side chain is protonated , more stable .
	manualset3
204227	8	417625	7	NULL	NULL	0	NULL	arginine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas unsolvated lithiated arginine is nonzwitterionic , these results provide compelling evidence that attachment of a single water molecule to this ion makes the zwitterionic form of arginine , in which the side chain is protonated , more stable .
	manualset3
204228	9	417625	7	NULL	NULL	0	NULL	 side chain	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas unsolvated lithiated arginine is nonzwitterionic , these results provide compelling evidence that attachment of a single water molecule to this ion makes the zwitterionic form of arginine , in which the side chain is protonated , more stable .
	manualset3
204232	1	417626	7	NULL	NULL	NULL	NULL	conduction	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Whether conduction in the long fiber tracts of the spinal cord can be similarly modulated is unknown .
	manualset3
204233	2	417626	7	NULL	NULL	0	NULL	long fiber tracts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether conduction in the long fiber tracts of the spinal cord can be similarly modulated is unknown .
	manualset3
204234	3	417626	7	NULL	NULL	0	NULL	spinal cord	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether conduction in the long fiber tracts of the spinal cord can be similarly modulated is unknown .
	manualset3
204235	1	417627	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients had an active duodenal ulcer confirmed by either endoscopy and/or surgery .
	manualset3
204236	2	417627	7	NULL	NULL	0	NULL	active duodenal ulcer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients had an active duodenal ulcer confirmed by either endoscopy and/or surgery .
	manualset3
204237	3	417627	7	NULL	NULL	0	NULL	endoscopy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients had an active duodenal ulcer confirmed by either endoscopy and/or surgery .
	manualset3
204238	4	417627	7	NULL	NULL	0	NULL	 surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients had an active duodenal ulcer confirmed by either endoscopy and/or surgery .
	manualset3
204239	1	417628	7	NULL	NULL	0	NULL	recurrences	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether recurrences of nasopharyngeal angiofibromas in some way is related to the amount and composition of the vascular components was studied by estimating the volume densities of the vascular lumen , the wall of thin-walled ( lined only with endothelial cells ) and thick-walled vessels ( several cell-layers in the vascular wall ) in seven cases of recurring and five non-recurring tumors .
	manualset3
204240	2	417628	7	NULL	NULL	0	NULL	nasopharyngeal angiofibromas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether recurrences of nasopharyngeal angiofibromas in some way is related to the amount and composition of the vascular components was studied by estimating the volume densities of the vascular lumen , the wall of thin-walled ( lined only with endothelial cells ) and thick-walled vessels ( several cell-layers in the vascular wall ) in seven cases of recurring and five non-recurring tumors .
	manualset3
204241	3	417628	7	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether recurrences of nasopharyngeal angiofibromas in some way is related to the amount and composition of the vascular components was studied by estimating the volume densities of the vascular lumen , the wall of thin-walled ( lined only with endothelial cells ) and thick-walled vessels ( several cell-layers in the vascular wall ) in seven cases of recurring and five non-recurring tumors .
	manualset3
204242	4	417628	7	NULL	NULL	0	NULL	composition	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether recurrences of nasopharyngeal angiofibromas in some way is related to the amount and composition of the vascular components was studied by estimating the volume densities of the vascular lumen , the wall of thin-walled ( lined only with endothelial cells ) and thick-walled vessels ( several cell-layers in the vascular wall ) in seven cases of recurring and five non-recurring tumors .
	manualset3
204243	5	417628	7	NULL	NULL	0	NULL	vascular components	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether recurrences of nasopharyngeal angiofibromas in some way is related to the amount and composition of the vascular components was studied by estimating the volume densities of the vascular lumen , the wall of thin-walled ( lined only with endothelial cells ) and thick-walled vessels ( several cell-layers in the vascular wall ) in seven cases of recurring and five non-recurring tumors .
	manualset3
204244	6	417628	7	NULL	NULL	0	NULL	volume densities	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether recurrences of nasopharyngeal angiofibromas in some way is related to the amount and composition of the vascular components was studied by estimating the volume densities of the vascular lumen , the wall of thin-walled ( lined only with endothelial cells ) and thick-walled vessels ( several cell-layers in the vascular wall ) in seven cases of recurring and five non-recurring tumors .
	manualset3
204245	7	417628	7	NULL	NULL	0	NULL	vascular lumen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether recurrences of nasopharyngeal angiofibromas in some way is related to the amount and composition of the vascular components was studied by estimating the volume densities of the vascular lumen , the wall of thin-walled ( lined only with endothelial cells ) and thick-walled vessels ( several cell-layers in the vascular wall ) in seven cases of recurring and five non-recurring tumors .
	manualset3
204246	8	417628	7	NULL	NULL	NULL	NULL	wall	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Whether recurrences of nasopharyngeal angiofibromas in some way is related to the amount and composition of the vascular components was studied by estimating the volume densities of the vascular lumen , the wall of thin-walled ( lined only with endothelial cells ) and thick-walled vessels ( several cell-layers in the vascular wall ) in seven cases of recurring and five non-recurring tumors .
	manualset3
204247	9	417628	7	NULL	NULL	0	NULL	thin-walled vessels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether recurrences of nasopharyngeal angiofibromas in some way is related to the amount and composition of the vascular components was studied by estimating the volume densities of the vascular lumen , the wall of thin-walled ( lined only with endothelial cells ) and thick-walled vessels ( several cell-layers in the vascular wall ) in seven cases of recurring and five non-recurring tumors .
	manualset3
204248	10	417628	7	NULL	NULL	0	NULL	endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether recurrences of nasopharyngeal angiofibromas in some way is related to the amount and composition of the vascular components was studied by estimating the volume densities of the vascular lumen , the wall of thin-walled ( lined only with endothelial cells ) and thick-walled vessels ( several cell-layers in the vascular wall ) in seven cases of recurring and five non-recurring tumors .
	manualset3
204249	11	417628	7	NULL	NULL	0	NULL	thick-walled vessels 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether recurrences of nasopharyngeal angiofibromas in some way is related to the amount and composition of the vascular components was studied by estimating the volume densities of the vascular lumen , the wall of thin-walled ( lined only with endothelial cells ) and thick-walled vessels ( several cell-layers in the vascular wall ) in seven cases of recurring and five non-recurring tumors .
	manualset3
204250	12	417628	7	NULL	NULL	0	NULL	cell-layers	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether recurrences of nasopharyngeal angiofibromas in some way is related to the amount and composition of the vascular components was studied by estimating the volume densities of the vascular lumen , the wall of thin-walled ( lined only with endothelial cells ) and thick-walled vessels ( several cell-layers in the vascular wall ) in seven cases of recurring and five non-recurring tumors .
	manualset3
204251	13	417628	7	NULL	NULL	0	NULL	vascular wall	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether recurrences of nasopharyngeal angiofibromas in some way is related to the amount and composition of the vascular components was studied by estimating the volume densities of the vascular lumen , the wall of thin-walled ( lined only with endothelial cells ) and thick-walled vessels ( several cell-layers in the vascular wall ) in seven cases of recurring and five non-recurring tumors .
	manualset3
204252	14	417628	7	NULL	NULL	0	NULL	seven cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether recurrences of nasopharyngeal angiofibromas in some way is related to the amount and composition of the vascular components was studied by estimating the volume densities of the vascular lumen , the wall of thin-walled ( lined only with endothelial cells ) and thick-walled vessels ( several cell-layers in the vascular wall ) in seven cases of recurring and five non-recurring tumors .
	manualset3
204253	15	417628	7	NULL	NULL	0	NULL	five non-recurring tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether recurrences of nasopharyngeal angiofibromas in some way is related to the amount and composition of the vascular components was studied by estimating the volume densities of the vascular lumen , the wall of thin-walled ( lined only with endothelial cells ) and thick-walled vessels ( several cell-layers in the vascular wall ) in seven cases of recurring and five non-recurring tumors .
	manualset3
204256	1	417629	7	NULL	NULL	0	NULL	plaque inhibition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether the plaque inhibition obtained with Triclosan/zinc citrate toothpaste was greater than would be expected from other commercially available preparations can not be determined from this study and is the subject of a further investigation .
	manualset3
204257	2	417629	7	NULL	NULL	0	NULL	Triclosan/zinc citrate toothpaste	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether the plaque inhibition obtained with Triclosan/zinc citrate toothpaste was greater than would be expected from other commercially available preparations can not be determined from this study and is the subject of a further investigation .
	manualset3
204259	3	417629	7	NULL	NULL	0	NULL	preparations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether the plaque inhibition obtained with Triclosan/zinc citrate toothpaste was greater than would be expected from other commercially available preparations can not be determined from this study and is the subject of a further investigation .
	manualset3
204260	4	417629	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether the plaque inhibition obtained with Triclosan/zinc citrate toothpaste was greater than would be expected from other commercially available preparations can not be determined from this study and is the subject of a further investigation .
	manualset3
204262	5	417629	7	NULL	NULL	0	NULL	subject	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether the plaque inhibition obtained with Triclosan/zinc citrate toothpaste was greater than would be expected from other commercially available preparations can not be determined from this study and is the subject of a further investigation .
	manualset3
204263	6	417629	7	NULL	NULL	0	NULL	investigation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether the plaque inhibition obtained with Triclosan/zinc citrate toothpaste was greater than would be expected from other commercially available preparations can not be determined from this study and is the subject of a further investigation .
	manualset3
204274	1	417630	7	NULL	NULL	0	NULL	inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether this inhibition is diffuse or specific for saccade direction is not known .
	manualset3
204276	2	417630	7	NULL	NULL	0	NULL	saccade direction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether this inhibition is diffuse or specific for saccade direction is not known .
	manualset3
204277	1	417631	7	NULL	NULL	0	NULL	organelle 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether or not an organelle is formed in the cell body might determine directionality .
	manualset3
204278	2	417631	7	NULL	NULL	0	NULL	cell body	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether or not an organelle is formed in the cell body might determine directionality .
	manualset3
205516	3	417631	7	NULL	NULL	0	NULL	directionality	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether or not an organelle is formed in the cell body might determine directionality .
	manualset3
204279	1	417632	7	NULL	NULL	0	NULL	spirituality	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether acknowledged or not , spirituality is part of the human condition of physicians as well as patients , and of the distinctive work that doctors do .
	manualset3
204280	2	417632	7	NULL	NULL	0	NULL	human condition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether acknowledged or not , spirituality is part of the human condition of physicians as well as patients , and of the distinctive work that doctors do .
	manualset3
204281	3	417632	7	NULL	NULL	0	NULL	physicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether acknowledged or not , spirituality is part of the human condition of physicians as well as patients , and of the distinctive work that doctors do .
	manualset3
204282	4	417632	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether acknowledged or not , spirituality is part of the human condition of physicians as well as patients , and of the distinctive work that doctors do .
	manualset3
204284	5	417632	7	NULL	NULL	NULL	NULL	doctors	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Whether acknowledged or not , spirituality is part of the human condition of physicians as well as patients , and of the distinctive work that doctors do .
	manualset3
205517	6	417632	7	NULL	NULL	0	NULL	distinctive work 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether acknowledged or not , spirituality is part of the human condition of physicians as well as patients , and of the distinctive work that doctors do .
	manualset3
204487	1	417633	7	NULL	NULL	0	NULL	region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Which is dominant depends on the region within the sinus node and the condition of the SNS .
	manualset3
204488	2	417633	7	NULL	NULL	0	NULL	sinus node	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Which is dominant depends on the region within the sinus node and the condition of the SNS .
	manualset3
204489	3	417633	7	NULL	NULL	0	NULL	condition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Which is dominant depends on the region within the sinus node and the condition of the SNS .
	manualset3
204490	4	417633	7	NULL	NULL	0	NULL	SNS	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Which is dominant depends on the region within the sinus node and the condition of the SNS .
	manualset3
204491	1	417634	7	NULL	NULL	0	NULL	radionuclides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Which radionuclides will nuclear oncology need tomorrow ?
	manualset3
204492	2	417634	7	NULL	NULL	0	NULL	nuclear oncology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Which radionuclides will nuclear oncology need tomorrow ?
	manualset3
204493	3	417634	7	NULL	NULL	0	NULL	tomorrow 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Which radionuclides will nuclear oncology need tomorrow ?
	manualset3
204494	1	417635	7	NULL	NULL	0	NULL	1 , 9-dimethylfluorene 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While 1 , 9-dimethylfluorene exhibited weak tumorigenic activity when administered by subcutaneous injection to newborn mice , 1-methylfluorene and 9-methylfluorene were inactive .
	manualset3
204495	2	417635	7	NULL	NULL	0	NULL	weak tumorigenic activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While 1 , 9-dimethylfluorene exhibited weak tumorigenic activity when administered by subcutaneous injection to newborn mice , 1-methylfluorene and 9-methylfluorene were inactive .
	manualset3
204496	3	417635	7	NULL	NULL	0	NULL	subcutaneous injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	While 1 , 9-dimethylfluorene exhibited weak tumorigenic activity when administered by subcutaneous injection to newborn mice , 1-methylfluorene and 9-methylfluorene were inactive .
	manualset3
204497	4	417635	7	NULL	NULL	0	NULL	newborn mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	While 1 , 9-dimethylfluorene exhibited weak tumorigenic activity when administered by subcutaneous injection to newborn mice , 1-methylfluorene and 9-methylfluorene were inactive .
	manualset3
204498	5	417635	7	NULL	NULL	0	NULL	 1-methylfluorene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While 1 , 9-dimethylfluorene exhibited weak tumorigenic activity when administered by subcutaneous injection to newborn mice , 1-methylfluorene and 9-methylfluorene were inactive .
	manualset3
204499	6	417635	7	NULL	NULL	0	NULL	 9-methylfluorene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While 1 , 9-dimethylfluorene exhibited weak tumorigenic activity when administered by subcutaneous injection to newborn mice , 1-methylfluorene and 9-methylfluorene were inactive .
	manualset3
204500	1	417636	7	NULL	NULL	0	NULL	 3 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	While 3 to 100 mg/kg of TRH reduced pentobarbital sleeping time when administered prior to the barbiturate , a dose-response relationship to TRH could not be established .
	manualset3
204501	2	417636	7	NULL	NULL	0	NULL	100 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	While 3 to 100 mg/kg of TRH reduced pentobarbital sleeping time when administered prior to the barbiturate , a dose-response relationship to TRH could not be established .
	manualset3
204502	3	417636	7	NULL	NULL	0	NULL	TRH	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While 3 to 100 mg/kg of TRH reduced pentobarbital sleeping time when administered prior to the barbiturate , a dose-response relationship to TRH could not be established .
	manualset3
204503	4	417636	7	NULL	NULL	0	NULL	pentobarbital sleeping time	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While 3 to 100 mg/kg of TRH reduced pentobarbital sleeping time when administered prior to the barbiturate , a dose-response relationship to TRH could not be established .
	manualset3
204504	5	417636	7	NULL	NULL	0	NULL	barbiturate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While 3 to 100 mg/kg of TRH reduced pentobarbital sleeping time when administered prior to the barbiturate , a dose-response relationship to TRH could not be established .
	manualset3
204505	6	417636	7	NULL	NULL	0	NULL	dose-response relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	While 3 to 100 mg/kg of TRH reduced pentobarbital sleeping time when administered prior to the barbiturate , a dose-response relationship to TRH could not be established .
	manualset3
204506	7	417636	7	NULL	NULL	0	NULL	TRH	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While 3 to 100 mg/kg of TRH reduced pentobarbital sleeping time when administered prior to the barbiturate , a dose-response relationship to TRH could not be established .
	manualset3
204507	1	417637	7	NULL	NULL	0	NULL	AV junction ablation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	While AV junction ablation and AV node modification can palliate some of the symptoms of atrial fibrillation by a control of ventricular rate , the arrhythmia persists with the loss of AV synchrony and continued risk of thromboembolism .
	manualset3
204508	2	417637	7	NULL	NULL	0	NULL	AV node modification	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	While AV junction ablation and AV node modification can palliate some of the symptoms of atrial fibrillation by a control of ventricular rate , the arrhythmia persists with the loss of AV synchrony and continued risk of thromboembolism .
	manualset3
204509	3	417637	7	NULL	NULL	0	NULL	symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While AV junction ablation and AV node modification can palliate some of the symptoms of atrial fibrillation by a control of ventricular rate , the arrhythmia persists with the loss of AV synchrony and continued risk of thromboembolism .
	manualset3
204510	4	417637	7	NULL	NULL	0	NULL	atrial fibrillation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While AV junction ablation and AV node modification can palliate some of the symptoms of atrial fibrillation by a control of ventricular rate , the arrhythmia persists with the loss of AV synchrony and continued risk of thromboembolism .
	manualset3
204511	5	417637	7	NULL	NULL	0	NULL	 control 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While AV junction ablation and AV node modification can palliate some of the symptoms of atrial fibrillation by a control of ventricular rate , the arrhythmia persists with the loss of AV synchrony and continued risk of thromboembolism .
	manualset3
204512	6	417637	7	NULL	NULL	0	NULL	ventricular rate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While AV junction ablation and AV node modification can palliate some of the symptoms of atrial fibrillation by a control of ventricular rate , the arrhythmia persists with the loss of AV synchrony and continued risk of thromboembolism .
	manualset3
204513	7	417637	7	NULL	NULL	0	NULL	arrhythmia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While AV junction ablation and AV node modification can palliate some of the symptoms of atrial fibrillation by a control of ventricular rate , the arrhythmia persists with the loss of AV synchrony and continued risk of thromboembolism .
	manualset3
204514	8	417637	7	NULL	NULL	0	NULL	loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While AV junction ablation and AV node modification can palliate some of the symptoms of atrial fibrillation by a control of ventricular rate , the arrhythmia persists with the loss of AV synchrony and continued risk of thromboembolism .
	manualset3
204515	9	417637	7	NULL	NULL	0	NULL	AV synchrony	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While AV junction ablation and AV node modification can palliate some of the symptoms of atrial fibrillation by a control of ventricular rate , the arrhythmia persists with the loss of AV synchrony and continued risk of thromboembolism .
	manualset3
204516	10	417637	7	NULL	NULL	0	NULL	 continued risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While AV junction ablation and AV node modification can palliate some of the symptoms of atrial fibrillation by a control of ventricular rate , the arrhythmia persists with the loss of AV synchrony and continued risk of thromboembolism .
	manualset3
204517	11	417637	7	NULL	NULL	0	NULL	thromboembolism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While AV junction ablation and AV node modification can palliate some of the symptoms of atrial fibrillation by a control of ventricular rate , the arrhythmia persists with the loss of AV synchrony and continued risk of thromboembolism .
	manualset3
204518	1	417638	7	NULL	NULL	0	NULL	CAT activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While CAT and POD activities increased with maturation , PPO activities decreased .
	manualset3
204519	2	417638	7	NULL	NULL	0	NULL	POD activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While CAT and POD activities increased with maturation , PPO activities decreased .
	manualset3
204520	3	417638	7	NULL	NULL	0	NULL	maturation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While CAT and POD activities increased with maturation , PPO activities decreased .
	manualset3
204521	4	417638	7	NULL	NULL	0	NULL	PPO activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While CAT and POD activities increased with maturation , PPO activities decreased .
	manualset3
204522	1	417639	7	NULL	NULL	0	NULL	 E2FB-RBR1 ( retinoblastoma-related protein 1 ) complexes	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	While E2FB-RBR1 ( retinoblastoma-related protein 1 ) complexes are reduced after sucrose addition or at elevated CYCD3 ; 1 levels , E2FA maintains a stable complex with RBR1 in proliferating cells .
	manualset3
204523	2	417639	7	NULL	NULL	0	NULL	sucrose addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While E2FB-RBR1 ( retinoblastoma-related protein 1 ) complexes are reduced after sucrose addition or at elevated CYCD3 ; 1 levels , E2FA maintains a stable complex with RBR1 in proliferating cells .
	manualset3
204524	3	417639	7	NULL	NULL	0	NULL	elevated CYCD3	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While E2FB-RBR1 ( retinoblastoma-related protein 1 ) complexes are reduced after sucrose addition or at elevated CYCD3 ; 1 levels , E2FA maintains a stable complex with RBR1 in proliferating cells .
	manualset3
204525	4	417639	7	NULL	NULL	0	NULL	1 levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While E2FB-RBR1 ( retinoblastoma-related protein 1 ) complexes are reduced after sucrose addition or at elevated CYCD3 ; 1 levels , E2FA maintains a stable complex with RBR1 in proliferating cells .
	manualset3
204526	5	417639	7	NULL	NULL	0	NULL	E2FA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	While E2FB-RBR1 ( retinoblastoma-related protein 1 ) complexes are reduced after sucrose addition or at elevated CYCD3 ; 1 levels , E2FA maintains a stable complex with RBR1 in proliferating cells .
	manualset3
204527	6	417639	7	NULL	NULL	0	NULL	stable complex	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	While E2FB-RBR1 ( retinoblastoma-related protein 1 ) complexes are reduced after sucrose addition or at elevated CYCD3 ; 1 levels , E2FA maintains a stable complex with RBR1 in proliferating cells .
	manualset3
204528	7	417639	7	NULL	NULL	0	NULL	RBR1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	While E2FB-RBR1 ( retinoblastoma-related protein 1 ) complexes are reduced after sucrose addition or at elevated CYCD3 ; 1 levels , E2FA maintains a stable complex with RBR1 in proliferating cells .
	manualset3
204529	8	417639	7	NULL	NULL	0	NULL	proliferating cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	While E2FB-RBR1 ( retinoblastoma-related protein 1 ) complexes are reduced after sucrose addition or at elevated CYCD3 ; 1 levels , E2FA maintains a stable complex with RBR1 in proliferating cells .
	manualset3
204530	1	417640	7	NULL	NULL	0	NULL	SeMet treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	While SeMet treatment led to accumulation within embryos , selenium concentrations were unaltered by salinity treatment .
	manualset3
204531	2	417640	7	NULL	NULL	0	NULL	accumulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While SeMet treatment led to accumulation within embryos , selenium concentrations were unaltered by salinity treatment .
	manualset3
204532	3	417640	7	NULL	NULL	0	NULL	embryos	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	While SeMet treatment led to accumulation within embryos , selenium concentrations were unaltered by salinity treatment .
	manualset3
204533	4	417640	7	NULL	NULL	0	NULL	selenium concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While SeMet treatment led to accumulation within embryos , selenium concentrations were unaltered by salinity treatment .
	manualset3
204534	5	417640	7	NULL	NULL	0	NULL	salinity treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	While SeMet treatment led to accumulation within embryos , selenium concentrations were unaltered by salinity treatment .
	manualset3
204535	1	417641	7	NULL	NULL	0	NULL	Type III dissecting aneurysms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While Type III dissecting aneurysms of the aorta in patients with renal transplants have been described , this report appears to represent the first successful replacement of the ascending aorta with correction of valvar aortic insufficiency in a patient with a Type I aortic dissection .
	manualset3
204536	2	417641	7	NULL	NULL	0	NULL	aorta	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	While Type III dissecting aneurysms of the aorta in patients with renal transplants have been described , this report appears to represent the first successful replacement of the ascending aorta with correction of valvar aortic insufficiency in a patient with a Type I aortic dissection .
	manualset3
204537	3	417641	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	While Type III dissecting aneurysms of the aorta in patients with renal transplants have been described , this report appears to represent the first successful replacement of the ascending aorta with correction of valvar aortic insufficiency in a patient with a Type I aortic dissection .
	manualset3
204538	4	417641	7	NULL	NULL	0	NULL	renal transplants	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	While Type III dissecting aneurysms of the aorta in patients with renal transplants have been described , this report appears to represent the first successful replacement of the ascending aorta with correction of valvar aortic insufficiency in a patient with a Type I aortic dissection .
	manualset3
204539	5	417641	7	NULL	NULL	0	NULL	report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	While Type III dissecting aneurysms of the aorta in patients with renal transplants have been described , this report appears to represent the first successful replacement of the ascending aorta with correction of valvar aortic insufficiency in a patient with a Type I aortic dissection .
	manualset3
204540	6	417641	7	NULL	NULL	0	NULL	 first successful replacement	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	While Type III dissecting aneurysms of the aorta in patients with renal transplants have been described , this report appears to represent the first successful replacement of the ascending aorta with correction of valvar aortic insufficiency in a patient with a Type I aortic dissection .
	manualset3
204541	7	417641	7	NULL	NULL	0	NULL	ascending aorta	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	While Type III dissecting aneurysms of the aorta in patients with renal transplants have been described , this report appears to represent the first successful replacement of the ascending aorta with correction of valvar aortic insufficiency in a patient with a Type I aortic dissection .
	manualset3
204542	8	417641	7	NULL	NULL	0	NULL	correction 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While Type III dissecting aneurysms of the aorta in patients with renal transplants have been described , this report appears to represent the first successful replacement of the ascending aorta with correction of valvar aortic insufficiency in a patient with a Type I aortic dissection .
	manualset3
204543	9	417641	7	NULL	NULL	0	NULL	valvar aortic insufficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While Type III dissecting aneurysms of the aorta in patients with renal transplants have been described , this report appears to represent the first successful replacement of the ascending aorta with correction of valvar aortic insufficiency in a patient with a Type I aortic dissection .
	manualset3
204544	10	417641	7	NULL	NULL	0	NULL	 patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	While Type III dissecting aneurysms of the aorta in patients with renal transplants have been described , this report appears to represent the first successful replacement of the ascending aorta with correction of valvar aortic insufficiency in a patient with a Type I aortic dissection .
	manualset3
204545	11	417641	7	NULL	NULL	0	NULL	Type I aortic dissection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While Type III dissecting aneurysms of the aorta in patients with renal transplants have been described , this report appears to represent the first successful replacement of the ascending aorta with correction of valvar aortic insufficiency in a patient with a Type I aortic dissection .
	manualset3
204546	1	417642	7	NULL	NULL	0	NULL	aged Rasgrp1 - / - mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	While aged Rasgrp1 - / - mice develop late-onset autoimmunity characterized by splenomegaly and the presence of anti-nuclear antibodies ( ANA ) , the additional loss of RasGRP3 expression inhibits this phenotype .
	manualset3
204547	2	417642	7	NULL	NULL	0	NULL	late-onset autoimmunity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While aged Rasgrp1 - / - mice develop late-onset autoimmunity characterized by splenomegaly and the presence of anti-nuclear antibodies ( ANA ) , the additional loss of RasGRP3 expression inhibits this phenotype .
	manualset3
204548	3	417642	7	NULL	NULL	0	NULL	splenomegaly	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While aged Rasgrp1 - / - mice develop late-onset autoimmunity characterized by splenomegaly and the presence of anti-nuclear antibodies ( ANA ) , the additional loss of RasGRP3 expression inhibits this phenotype .
	manualset3
204549	4	417642	7	NULL	NULL	0	NULL	presence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While aged Rasgrp1 - / - mice develop late-onset autoimmunity characterized by splenomegaly and the presence of anti-nuclear antibodies ( ANA ) , the additional loss of RasGRP3 expression inhibits this phenotype .
	manualset3
204550	5	417642	7	NULL	NULL	0	NULL	anti-nuclear antibodies ( ANA )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	While aged Rasgrp1 - / - mice develop late-onset autoimmunity characterized by splenomegaly and the presence of anti-nuclear antibodies ( ANA ) , the additional loss of RasGRP3 expression inhibits this phenotype .
	manualset3
204551	6	417642	7	NULL	NULL	0	NULL	 loss 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While aged Rasgrp1 - / - mice develop late-onset autoimmunity characterized by splenomegaly and the presence of anti-nuclear antibodies ( ANA ) , the additional loss of RasGRP3 expression inhibits this phenotype .
	manualset3
204552	7	417642	7	NULL	NULL	0	NULL	RasGRP3 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While aged Rasgrp1 - / - mice develop late-onset autoimmunity characterized by splenomegaly and the presence of anti-nuclear antibodies ( ANA ) , the additional loss of RasGRP3 expression inhibits this phenotype .
	manualset3
204553	8	417642	7	NULL	NULL	0	NULL	phenotype	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	While aged Rasgrp1 - / - mice develop late-onset autoimmunity characterized by splenomegaly and the presence of anti-nuclear antibodies ( ANA ) , the additional loss of RasGRP3 expression inhibits this phenotype .
	manualset3
204554	1	417643	7	NULL	NULL	0	NULL	biologists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	While always of importance to biologists , having numbers in hand is becoming increasingly critical for experimenting , modeling , and analyzing biological systems .
	manualset3
204555	2	417643	7	NULL	NULL	NULL	NULL	numbers in hand	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While always of importance to biologists , having numbers in hand is becoming increasingly critical for experimenting , modeling , and analyzing biological systems .
	manualset3
204556	4	417643	7	NULL	NULL	NULL	NULL	biological systems	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While always of importance to biologists , having numbers in hand is becoming increasingly critical for experimenting , modeling , and analyzing biological systems .
	manualset3
204558	1	417644	7	NULL	NULL	0	NULL	alkenes 20	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While both alkenes 20 and 39 failed to give the expected cyclobutane or diene dimers , 20 was reacted with 3 , 7-dimethyltricyclo ( 3.3.0.0 ( 3 , 7 ) ) oct-1 ( 5 ) - ene ( 1b ) to give the cross-coupled product 4 , 5 - ( 2 , 2 ' ) - biphenylene-10 , 11 - dimethylpentacyclo ( 8.2.1.1 ( 2 , 5 ) .1 ( 4 , 7 ) .1 ( 8 , 11 ) ) hexadeca-1 , 7 - diene ( 33 ) .
	manualset3
204559	2	417644	7	NULL	NULL	0	NULL	alkenes 39	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While both alkenes 20 and 39 failed to give the expected cyclobutane or diene dimers , 20 was reacted with 3 , 7-dimethyltricyclo ( 3.3.0.0 ( 3 , 7 ) ) oct-1 ( 5 ) - ene ( 1b ) to give the cross-coupled product 4 , 5 - ( 2 , 2 ' ) - biphenylene-10 , 11 - dimethylpentacyclo ( 8.2.1.1 ( 2 , 5 ) .1 ( 4 , 7 ) .1 ( 8 , 11 ) ) hexadeca-1 , 7 - diene ( 33 ) .
	manualset3
204560	3	417644	7	NULL	NULL	0	NULL	cyclobutane	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While both alkenes 20 and 39 failed to give the expected cyclobutane or diene dimers , 20 was reacted with 3 , 7-dimethyltricyclo ( 3.3.0.0 ( 3 , 7 ) ) oct-1 ( 5 ) - ene ( 1b ) to give the cross-coupled product 4 , 5 - ( 2 , 2 ' ) - biphenylene-10 , 11 - dimethylpentacyclo ( 8.2.1.1 ( 2 , 5 ) .1 ( 4 , 7 ) .1 ( 8 , 11 ) ) hexadeca-1 , 7 - diene ( 33 ) .
	manualset3
204561	4	417644	7	NULL	NULL	0	NULL	diene dimers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While both alkenes 20 and 39 failed to give the expected cyclobutane or diene dimers , 20 was reacted with 3 , 7-dimethyltricyclo ( 3.3.0.0 ( 3 , 7 ) ) oct-1 ( 5 ) - ene ( 1b ) to give the cross-coupled product 4 , 5 - ( 2 , 2 ' ) - biphenylene-10 , 11 - dimethylpentacyclo ( 8.2.1.1 ( 2 , 5 ) .1 ( 4 , 7 ) .1 ( 8 , 11 ) ) hexadeca-1 , 7 - diene ( 33 ) .
	manualset3
204562	5	417644	7	NULL	NULL	0	NULL	20	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While both alkenes 20 and 39 failed to give the expected cyclobutane or diene dimers , 20 was reacted with 3 , 7-dimethyltricyclo ( 3.3.0.0 ( 3 , 7 ) ) oct-1 ( 5 ) - ene ( 1b ) to give the cross-coupled product 4 , 5 - ( 2 , 2 ' ) - biphenylene-10 , 11 - dimethylpentacyclo ( 8.2.1.1 ( 2 , 5 ) .1 ( 4 , 7 ) .1 ( 8 , 11 ) ) hexadeca-1 , 7 - diene ( 33 ) .
	manualset3
204563	6	417644	7	NULL	NULL	0	NULL	 3 , 7-dimethyltricyclo ( 3.3.0.0 ( 3 , 7 ) ) oct-1 ( 5 ) - ene ( 1b )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While both alkenes 20 and 39 failed to give the expected cyclobutane or diene dimers , 20 was reacted with 3 , 7-dimethyltricyclo ( 3.3.0.0 ( 3 , 7 ) ) oct-1 ( 5 ) - ene ( 1b ) to give the cross-coupled product 4 , 5 - ( 2 , 2 ' ) - biphenylene-10 , 11 - dimethylpentacyclo ( 8.2.1.1 ( 2 , 5 ) .1 ( 4 , 7 ) .1 ( 8 , 11 ) ) hexadeca-1 , 7 - diene ( 33 ) .
	manualset3
204564	7	417644	7	NULL	NULL	0	NULL	cross-coupled product	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While both alkenes 20 and 39 failed to give the expected cyclobutane or diene dimers , 20 was reacted with 3 , 7-dimethyltricyclo ( 3.3.0.0 ( 3 , 7 ) ) oct-1 ( 5 ) - ene ( 1b ) to give the cross-coupled product 4 , 5 - ( 2 , 2 ' ) - biphenylene-10 , 11 - dimethylpentacyclo ( 8.2.1.1 ( 2 , 5 ) .1 ( 4 , 7 ) .1 ( 8 , 11 ) ) hexadeca-1 , 7 - diene ( 33 ) .
	manualset3
204565	8	417644	7	NULL	NULL	0	NULL	4 , 5 - ( 2 , 2 ' ) - biphenylene-10 , 11 - dimethylpentacyclo ( 8.2.1.1 ( 2 , 5 ) .1 ( 4 , 7 ) .1 ( 8 , 11 ) ) hexadeca-1 , 7 - diene ( 33 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While both alkenes 20 and 39 failed to give the expected cyclobutane or diene dimers , 20 was reacted with 3 , 7-dimethyltricyclo ( 3.3.0.0 ( 3 , 7 ) ) oct-1 ( 5 ) - ene ( 1b ) to give the cross-coupled product 4 , 5 - ( 2 , 2 ' ) - biphenylene-10 , 11 - dimethylpentacyclo ( 8.2.1.1 ( 2 , 5 ) .1 ( 4 , 7 ) .1 ( 8 , 11 ) ) hexadeca-1 , 7 - diene ( 33 ) .
	manualset3
204566	1	417645	7	NULL	NULL	0	NULL	caregiver	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	While caregiver and youth motivations correlate , their agreement is low .
	manualset3
204567	2	417645	7	NULL	NULL	0	NULL	youth motivations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While caregiver and youth motivations correlate , their agreement is low .
	manualset3
204568	3	417645	7	NULL	NULL	0	NULL	agreement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While caregiver and youth motivations correlate , their agreement is low .
	manualset3
204569	1	417646	7	NULL	NULL	0	NULL	cataract 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While cataract is responsible for nearly 20 million of the 45 million blind people in the world , the next major cause is trachoma which blinds 4.9 million individuals , mainly as a result of corneal scarring and vascularization .
	manualset3
204570	2	417646	7	NULL	NULL	0	NULL	20 million blind people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	While cataract is responsible for nearly 20 million of the 45 million blind people in the world , the next major cause is trachoma which blinds 4.9 million individuals , mainly as a result of corneal scarring and vascularization .
	manualset3
204571	3	417646	7	NULL	NULL	0	NULL	45 million blind people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	While cataract is responsible for nearly 20 million of the 45 million blind people in the world , the next major cause is trachoma which blinds 4.9 million individuals , mainly as a result of corneal scarring and vascularization .
	manualset3
204572	4	417646	7	NULL	NULL	0	NULL	world	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	While cataract is responsible for nearly 20 million of the 45 million blind people in the world , the next major cause is trachoma which blinds 4.9 million individuals , mainly as a result of corneal scarring and vascularization .
	manualset3
204573	5	417646	7	NULL	NULL	0	NULL	major cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While cataract is responsible for nearly 20 million of the 45 million blind people in the world , the next major cause is trachoma which blinds 4.9 million individuals , mainly as a result of corneal scarring and vascularization .
	manualset3
204574	6	417646	7	NULL	NULL	NULL	NULL	trachoma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While cataract is responsible for nearly 20 million of the 45 million blind people in the world , the next major cause is trachoma which blinds 4.9 million individuals , mainly as a result of corneal scarring and vascularization .
	manualset3
204575	7	417646	7	NULL	NULL	0	NULL	4.9 million individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	While cataract is responsible for nearly 20 million of the 45 million blind people in the world , the next major cause is trachoma which blinds 4.9 million individuals , mainly as a result of corneal scarring and vascularization .
	manualset3
204576	8	417646	7	NULL	NULL	0	NULL	result	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While cataract is responsible for nearly 20 million of the 45 million blind people in the world , the next major cause is trachoma which blinds 4.9 million individuals , mainly as a result of corneal scarring and vascularization .
	manualset3
204577	9	417646	7	NULL	NULL	0	NULL	corneal scarring	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While cataract is responsible for nearly 20 million of the 45 million blind people in the world , the next major cause is trachoma which blinds 4.9 million individuals , mainly as a result of corneal scarring and vascularization .
	manualset3
204578	10	417646	7	NULL	NULL	0	NULL	vascularization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While cataract is responsible for nearly 20 million of the 45 million blind people in the world , the next major cause is trachoma which blinds 4.9 million individuals , mainly as a result of corneal scarring and vascularization .
	manualset3
204579	1	417647	7	NULL	NULL	NULL	NULL	cause	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While clearly not establishing cause and effect , free radical-mediated changes in peripheral amino acid metabolism known to influence immune and cerebral serotoninergic function may enhance susceptibility to and/or delay recovery from altitude illness .
	manualset3
204580	2	417647	7	NULL	NULL	NULL	NULL	effect	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While clearly not establishing cause and effect , free radical-mediated changes in peripheral amino acid metabolism known to influence immune and cerebral serotoninergic function may enhance susceptibility to and/or delay recovery from altitude illness .
	manualset3
204581	3	417647	7	NULL	NULL	0	NULL	free radical-mediated changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While clearly not establishing cause and effect , free radical-mediated changes in peripheral amino acid metabolism known to influence immune and cerebral serotoninergic function may enhance susceptibility to and/or delay recovery from altitude illness .
	manualset3
204582	4	417647	7	NULL	NULL	0	NULL	peripheral amino acid metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While clearly not establishing cause and effect , free radical-mediated changes in peripheral amino acid metabolism known to influence immune and cerebral serotoninergic function may enhance susceptibility to and/or delay recovery from altitude illness .
	manualset3
204583	5	417647	7	NULL	NULL	0	NULL	immune serotoninergic function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While clearly not establishing cause and effect , free radical-mediated changes in peripheral amino acid metabolism known to influence immune and cerebral serotoninergic function may enhance susceptibility to and/or delay recovery from altitude illness .
	manualset3
204584	6	417647	7	NULL	NULL	0	NULL	cerebral serotoninergic function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While clearly not establishing cause and effect , free radical-mediated changes in peripheral amino acid metabolism known to influence immune and cerebral serotoninergic function may enhance susceptibility to and/or delay recovery from altitude illness .
	manualset3
204585	7	417647	7	NULL	NULL	NULL	NULL	susceptibility	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While clearly not establishing cause and effect , free radical-mediated changes in peripheral amino acid metabolism known to influence immune and cerebral serotoninergic function may enhance susceptibility to and/or delay recovery from altitude illness .
	manualset3
204586	8	417647	7	NULL	NULL	0	NULL	delay recovery	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While clearly not establishing cause and effect , free radical-mediated changes in peripheral amino acid metabolism known to influence immune and cerebral serotoninergic function may enhance susceptibility to and/or delay recovery from altitude illness .
	manualset3
204587	9	417647	7	NULL	NULL	0	NULL	altitude illness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While clearly not establishing cause and effect , free radical-mediated changes in peripheral amino acid metabolism known to influence immune and cerebral serotoninergic function may enhance susceptibility to and/or delay recovery from altitude illness .
	manualset3
204588	1	417648	7	NULL	NULL	0	NULL	cleavage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While cleavage away from the cyano group is preferred kinetically , cleavage adjacent to the cyano group is preferred thermodynamically .
	manualset3
204589	2	417648	7	NULL	NULL	0	NULL	cyano group	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While cleavage away from the cyano group is preferred kinetically , cleavage adjacent to the cyano group is preferred thermodynamically .
	manualset3
204590	3	417648	7	NULL	NULL	0	NULL	cleavage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While cleavage away from the cyano group is preferred kinetically , cleavage adjacent to the cyano group is preferred thermodynamically .
	manualset3
204591	4	417648	7	NULL	NULL	0	NULL	cyano group	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While cleavage away from the cyano group is preferred kinetically , cleavage adjacent to the cyano group is preferred thermodynamically .
	manualset3
204592	1	417649	7	NULL	NULL	0	NULL	clinical studies testing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While clinical studies testing this new approach are about to start , the development of other novel therapeutic approaches is greatly hampered by the lack of sufficient animal models of IgAN .
	manualset3
204593	2	417649	7	NULL	NULL	0	NULL	new approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While clinical studies testing this new approach are about to start , the development of other novel therapeutic approaches is greatly hampered by the lack of sufficient animal models of IgAN .
	manualset3
204594	3	417649	7	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While clinical studies testing this new approach are about to start , the development of other novel therapeutic approaches is greatly hampered by the lack of sufficient animal models of IgAN .
	manualset3
204595	4	417649	7	NULL	NULL	0	NULL	novel therapeutic approaches	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While clinical studies testing this new approach are about to start , the development of other novel therapeutic approaches is greatly hampered by the lack of sufficient animal models of IgAN .
	manualset3
204596	5	417649	7	NULL	NULL	0	NULL	 lack	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While clinical studies testing this new approach are about to start , the development of other novel therapeutic approaches is greatly hampered by the lack of sufficient animal models of IgAN .
	manualset3
204597	6	417649	7	NULL	NULL	0	NULL	animal models	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	While clinical studies testing this new approach are about to start , the development of other novel therapeutic approaches is greatly hampered by the lack of sufficient animal models of IgAN .
	manualset3
204598	7	417649	7	NULL	NULL	0	NULL	IgAN 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	While clinical studies testing this new approach are about to start , the development of other novel therapeutic approaches is greatly hampered by the lack of sufficient animal models of IgAN .
	manualset3
204599	1	417650	7	NULL	NULL	0	NULL	RN/BSN program	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	While designing an RN/BSN program , a small group of faculty accepted the challenge of the National League for Nursing ( NLN ) to initiate flexible , innovative learning experiences .
	manualset3
204600	2	417650	7	NULL	NULL	0	NULL	small group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	While designing an RN/BSN program , a small group of faculty accepted the challenge of the National League for Nursing ( NLN ) to initiate flexible , innovative learning experiences .
	manualset3
204601	3	417650	7	NULL	NULL	0	NULL	faculty	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	While designing an RN/BSN program , a small group of faculty accepted the challenge of the National League for Nursing ( NLN ) to initiate flexible , innovative learning experiences .
	manualset3
204602	4	417650	7	NULL	NULL	0	NULL	challenge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While designing an RN/BSN program , a small group of faculty accepted the challenge of the National League for Nursing ( NLN ) to initiate flexible , innovative learning experiences .
	manualset3
204603	5	417650	7	NULL	NULL	0	NULL	National League for Nursing ( NLN )	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	While designing an RN/BSN program , a small group of faculty accepted the challenge of the National League for Nursing ( NLN ) to initiate flexible , innovative learning experiences .
	manualset3
204604	6	417650	7	NULL	NULL	0	NULL	innovative learning experiences	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While designing an RN/BSN program , a small group of faculty accepted the challenge of the National League for Nursing ( NLN ) to initiate flexible , innovative learning experiences .
	manualset3
204605	1	417651	7	NULL	NULL	0	NULL	efforts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While earlier efforts relied upon approximations of keystroke efficiency , the proposed approach optimizes the arrangement under this exact performance measure .
	manualset3
204606	2	417651	7	NULL	NULL	0	NULL	approximations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While earlier efforts relied upon approximations of keystroke efficiency , the proposed approach optimizes the arrangement under this exact performance measure .
	manualset3
204607	3	417651	7	NULL	NULL	0	NULL	keystroke efficiency	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While earlier efforts relied upon approximations of keystroke efficiency , the proposed approach optimizes the arrangement under this exact performance measure .
	manualset3
204608	4	417651	7	NULL	NULL	0	NULL	proposed approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While earlier efforts relied upon approximations of keystroke efficiency , the proposed approach optimizes the arrangement under this exact performance measure .
	manualset3
204609	5	417651	7	NULL	NULL	0	NULL	arrangement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While earlier efforts relied upon approximations of keystroke efficiency , the proposed approach optimizes the arrangement under this exact performance measure .
	manualset3
204610	6	417651	7	NULL	NULL	0	NULL	exact performance measure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While earlier efforts relied upon approximations of keystroke efficiency , the proposed approach optimizes the arrangement under this exact performance measure .
	manualset3
204611	1	417652	7	NULL	NULL	0	NULL	endoscopic surveillance	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	While frequent endoscopic surveillance is acceptable , a case of early malignant transformation is presented , and the argument for prophylactic preemptive pancreaticoduodenectomy is made .
	manualset3
204612	2	417652	7	NULL	NULL	0	NULL	case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While frequent endoscopic surveillance is acceptable , a case of early malignant transformation is presented , and the argument for prophylactic preemptive pancreaticoduodenectomy is made .
	manualset3
204613	3	417652	7	NULL	NULL	0	NULL	early malignant transformation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While frequent endoscopic surveillance is acceptable , a case of early malignant transformation is presented , and the argument for prophylactic preemptive pancreaticoduodenectomy is made .
	manualset3
204614	4	417652	7	NULL	NULL	0	NULL	argument	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While frequent endoscopic surveillance is acceptable , a case of early malignant transformation is presented , and the argument for prophylactic preemptive pancreaticoduodenectomy is made .
	manualset3
204615	5	417652	7	NULL	NULL	0	NULL	prophylactic preemptive pancreaticoduodenectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	While frequent endoscopic surveillance is acceptable , a case of early malignant transformation is presented , and the argument for prophylactic preemptive pancreaticoduodenectomy is made .
	manualset3
204616	1	417653	7	NULL	NULL	0	NULL	case 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While it is the case that initial tobacco use often escalates to compulsive use accompanied by tolerance and physical dependence , this is not usually observed with nicotine replacement therapies .
	manualset3
204617	2	417653	7	NULL	NULL	0	NULL	 tobacco use 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While it is the case that initial tobacco use often escalates to compulsive use accompanied by tolerance and physical dependence , this is not usually observed with nicotine replacement therapies .
	manualset3
204618	3	417653	7	NULL	NULL	0	NULL	tolerance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While it is the case that initial tobacco use often escalates to compulsive use accompanied by tolerance and physical dependence , this is not usually observed with nicotine replacement therapies .
	manualset3
204619	4	417653	7	NULL	NULL	0	NULL	physical dependence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While it is the case that initial tobacco use often escalates to compulsive use accompanied by tolerance and physical dependence , this is not usually observed with nicotine replacement therapies .
	manualset3
204620	5	417653	7	NULL	NULL	0	NULL	nicotine replacement therapies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	While it is the case that initial tobacco use often escalates to compulsive use accompanied by tolerance and physical dependence , this is not usually observed with nicotine replacement therapies .
	manualset3
204621	1	417654	7	NULL	NULL	0	NULL	reduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While it is widely agreed that reduction of immunosuppression should be the first intervention after diagnosis of BKV infection , there is no consensus on whether calcineurin inhibitors or antiproliferative drugs should be reduced first .
	manualset3
204622	2	417654	7	NULL	NULL	0	NULL	immunosuppression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While it is widely agreed that reduction of immunosuppression should be the first intervention after diagnosis of BKV infection , there is no consensus on whether calcineurin inhibitors or antiproliferative drugs should be reduced first .
	manualset3
204623	3	417654	7	NULL	NULL	0	NULL	first intervention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While it is widely agreed that reduction of immunosuppression should be the first intervention after diagnosis of BKV infection , there is no consensus on whether calcineurin inhibitors or antiproliferative drugs should be reduced first .
	manualset3
204624	4	417654	7	NULL	NULL	0	NULL	 diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While it is widely agreed that reduction of immunosuppression should be the first intervention after diagnosis of BKV infection , there is no consensus on whether calcineurin inhibitors or antiproliferative drugs should be reduced first .
	manualset3
204625	5	417654	7	NULL	NULL	0	NULL	BKV infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While it is widely agreed that reduction of immunosuppression should be the first intervention after diagnosis of BKV infection , there is no consensus on whether calcineurin inhibitors or antiproliferative drugs should be reduced first .
	manualset3
204626	6	417654	7	NULL	NULL	0	NULL	consensus	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While it is widely agreed that reduction of immunosuppression should be the first intervention after diagnosis of BKV infection , there is no consensus on whether calcineurin inhibitors or antiproliferative drugs should be reduced first .
	manualset3
204627	7	417654	7	NULL	NULL	0	NULL	calcineurin inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While it is widely agreed that reduction of immunosuppression should be the first intervention after diagnosis of BKV infection , there is no consensus on whether calcineurin inhibitors or antiproliferative drugs should be reduced first .
	manualset3
204628	8	417654	7	NULL	NULL	0	NULL	antiproliferative drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	While it is widely agreed that reduction of immunosuppression should be the first intervention after diagnosis of BKV infection , there is no consensus on whether calcineurin inhibitors or antiproliferative drugs should be reduced first .
	manualset3
204629	1	417655	7	NULL	NULL	0	NULL	spore inactivation techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While many spore inactivation techniques have been proven effective , electron beam ( EB ) irradiation has been frequently chosen to eradicate Bacillus spores .
	manualset3
204630	2	417655	7	NULL	NULL	0	NULL	electron beam ( EB ) irradiation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While many spore inactivation techniques have been proven effective , electron beam ( EB ) irradiation has been frequently chosen to eradicate Bacillus spores .
	manualset3
204631	3	417655	7	NULL	NULL	0	NULL	Bacillus spores	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	While many spore inactivation techniques have been proven effective , electron beam ( EB ) irradiation has been frequently chosen to eradicate Bacillus spores .
	manualset3
204632	1	417656	7	NULL	NULL	0	NULL	medical literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	While medical literature has sporadically reported on the emotional impact of adverse events on healthcare professionals , little has been documented on the implementation of support services following these events .
	manualset3
204633	2	417656	7	NULL	NULL	NULL	NULL	emotional impact	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While medical literature has sporadically reported on the emotional impact of adverse events on healthcare professionals , little has been documented on the implementation of support services following these events .
	manualset3
204634	3	417656	7	NULL	NULL	0	NULL	adverse events	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While medical literature has sporadically reported on the emotional impact of adverse events on healthcare professionals , little has been documented on the implementation of support services following these events .
	manualset3
204635	4	417656	7	NULL	NULL	0	NULL	healthcare professionals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	While medical literature has sporadically reported on the emotional impact of adverse events on healthcare professionals , little has been documented on the implementation of support services following these events .
	manualset3
204636	5	417656	7	NULL	NULL	0	NULL	implementation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While medical literature has sporadically reported on the emotional impact of adverse events on healthcare professionals , little has been documented on the implementation of support services following these events .
	manualset3
204637	6	417656	7	NULL	NULL	0	NULL	support services	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	While medical literature has sporadically reported on the emotional impact of adverse events on healthcare professionals , little has been documented on the implementation of support services following these events .
	manualset3
204638	7	417656	7	NULL	NULL	0	NULL	events	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While medical literature has sporadically reported on the emotional impact of adverse events on healthcare professionals , little has been documented on the implementation of support services following these events .
	manualset3
204639	1	417657	7	NULL	NULL	0	NULL	 mental health nurses	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	While mental health nurses may see themselves as promoting inclusion , the reality may be quite different .
	manualset3
204640	2	417657	7	NULL	NULL	0	NULL	inclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While mental health nurses may see themselves as promoting inclusion , the reality may be quite different .
	manualset3
204641	3	417657	7	NULL	NULL	0	NULL	reality	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While mental health nurses may see themselves as promoting inclusion , the reality may be quite different .
	manualset3
204642	1	417658	7	NULL	NULL	NULL	NULL	methadone	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While methadone has been available for over 50 years , its use in opiate dependence has overshadowed its use as an analgesic .
	manualset3
204643	2	417658	7	NULL	NULL	0	NULL	50 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	While methadone has been available for over 50 years , its use in opiate dependence has overshadowed its use as an analgesic .
	manualset3
204644	3	417658	7	NULL	NULL	0	NULL	opiate dependence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While methadone has been available for over 50 years , its use in opiate dependence has overshadowed its use as an analgesic .
	manualset3
204645	4	417658	7	NULL	NULL	0	NULL	analgesic	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	While methadone has been available for over 50 years , its use in opiate dependence has overshadowed its use as an analgesic .
	manualset3
204646	1	417659	7	NULL	NULL	0	NULL	 solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While monomeric in solution , JEV E assembles as an antiparallel dimer in the crystal lattice organized in a highly similar fashion as seen in cryo-electron microscopy models of mature flavivirus virions .
	manualset3
204647	2	417659	7	NULL	NULL	0	NULL	JEV E	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	While monomeric in solution , JEV E assembles as an antiparallel dimer in the crystal lattice organized in a highly similar fashion as seen in cryo-electron microscopy models of mature flavivirus virions .
	manualset3
204648	3	417659	7	NULL	NULL	0	NULL	antiparallel dimer	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	While monomeric in solution , JEV E assembles as an antiparallel dimer in the crystal lattice organized in a highly similar fashion as seen in cryo-electron microscopy models of mature flavivirus virions .
	manualset3
204649	4	417659	7	NULL	NULL	NULL	NULL	crystal lattice	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While monomeric in solution , JEV E assembles as an antiparallel dimer in the crystal lattice organized in a highly similar fashion as seen in cryo-electron microscopy models of mature flavivirus virions .
	manualset3
204650	5	417659	7	NULL	NULL	NULL	NULL	cryo-electron microscopy models	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While monomeric in solution , JEV E assembles as an antiparallel dimer in the crystal lattice organized in a highly similar fashion as seen in cryo-electron microscopy models of mature flavivirus virions .
	manualset3
204651	6	417659	7	NULL	NULL	0	NULL	mature flavivirus virions	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	While monomeric in solution , JEV E assembles as an antiparallel dimer in the crystal lattice organized in a highly similar fashion as seen in cryo-electron microscopy models of mature flavivirus virions .
	manualset3
204652	1	417660	7	NULL	NULL	0	NULL	drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	While most drugs lose their efficacy against arrhythmias associated with myocardial ischemia and reperfusion , dofetilide remains effective .
	manualset3
204653	2	417660	7	NULL	NULL	0	NULL	arrhythmias	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While most drugs lose their efficacy against arrhythmias associated with myocardial ischemia and reperfusion , dofetilide remains effective .
	manualset3
204654	3	417660	7	NULL	NULL	NULL	NULL	myocardial ischemia 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While most drugs lose their efficacy against arrhythmias associated with myocardial ischemia and reperfusion , dofetilide remains effective .
	manualset3
204655	4	417660	7	NULL	NULL	0	NULL	reperfusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	While most drugs lose their efficacy against arrhythmias associated with myocardial ischemia and reperfusion , dofetilide remains effective .
	manualset3
204656	5	417660	7	NULL	NULL	0	NULL	dofetilide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	While most drugs lose their efficacy against arrhythmias associated with myocardial ischemia and reperfusion , dofetilide remains effective .
	manualset3
204657	1	417661	7	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	While no correlation was found between CECs and clinical features , more studies in a larger patient sample size and advanced disease are necessary .
	manualset3
204658	2	417661	7	NULL	NULL	0	NULL	CECs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	While no correlation was found between CECs and clinical features , more studies in a larger patient sample size and advanced disease are necessary .
	manualset3
204659	3	417661	7	NULL	NULL	0	NULL	clinical features	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While no correlation was found between CECs and clinical features , more studies in a larger patient sample size and advanced disease are necessary .
	manualset3
204660	4	417661	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While no correlation was found between CECs and clinical features , more studies in a larger patient sample size and advanced disease are necessary .
	manualset3
204661	5	417661	7	NULL	NULL	0	NULL	patient sample size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While no correlation was found between CECs and clinical features , more studies in a larger patient sample size and advanced disease are necessary .
	manualset3
204662	6	417661	7	NULL	NULL	0	NULL	 disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	While no correlation was found between CECs and clinical features , more studies in a larger patient sample size and advanced disease are necessary .
	manualset3
204663	1	417662	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients presented with abdominal distention , stunted growth , raised jugular venous pressure , ascites and hepatosplenomegaly .
	manualset3
204664	2	417662	7	NULL	NULL	0	NULL	abdominal distention	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients presented with abdominal distention , stunted growth , raised jugular venous pressure , ascites and hepatosplenomegaly .
	manualset3
204665	3	417662	7	NULL	NULL	0	NULL	stunted growth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients presented with abdominal distention , stunted growth , raised jugular venous pressure , ascites and hepatosplenomegaly .
	manualset3
204666	4	417662	7	NULL	NULL	NULL	NULL	raised jugular venous pressure	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	All patients presented with abdominal distention , stunted growth , raised jugular venous pressure , ascites and hepatosplenomegaly .
	manualset3
204667	5	417662	7	NULL	NULL	0	NULL	ascites	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients presented with abdominal distention , stunted growth , raised jugular venous pressure , ascites and hepatosplenomegaly .
	manualset3
204668	6	417662	7	NULL	NULL	0	NULL	 hepatosplenomegaly	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients presented with abdominal distention , stunted growth , raised jugular venous pressure , ascites and hepatosplenomegaly .
	manualset3
204669	1	417663	7	NULL	NULL	0	NULL	mouse MCAO models	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	While producing mouse MCAO models using commercially available silicone-coated monofilaments , we temporarily occluded the common carotid artery ( CCA ) or PPA to determine whether cerebral blood flow ( CBF ) values , infarct size and the stability of the model would be affected .
	manualset3
204670	2	417663	7	NULL	NULL	0	NULL	silicone-coated monofilaments	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While producing mouse MCAO models using commercially available silicone-coated monofilaments , we temporarily occluded the common carotid artery ( CCA ) or PPA to determine whether cerebral blood flow ( CBF ) values , infarct size and the stability of the model would be affected .
	manualset3
204671	3	417663	7	NULL	NULL	0	NULL	common carotid artery ( CCA ) 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	While producing mouse MCAO models using commercially available silicone-coated monofilaments , we temporarily occluded the common carotid artery ( CCA ) or PPA to determine whether cerebral blood flow ( CBF ) values , infarct size and the stability of the model would be affected .
	manualset3
204672	4	417663	7	NULL	NULL	0	NULL	PPA	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	While producing mouse MCAO models using commercially available silicone-coated monofilaments , we temporarily occluded the common carotid artery ( CCA ) or PPA to determine whether cerebral blood flow ( CBF ) values , infarct size and the stability of the model would be affected .
	manualset3
204673	5	417663	7	NULL	NULL	0	NULL	cerebral blood flow ( CBF ) values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While producing mouse MCAO models using commercially available silicone-coated monofilaments , we temporarily occluded the common carotid artery ( CCA ) or PPA to determine whether cerebral blood flow ( CBF ) values , infarct size and the stability of the model would be affected .
	manualset3
204674	6	417663	7	NULL	NULL	0	NULL	infarct size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While producing mouse MCAO models using commercially available silicone-coated monofilaments , we temporarily occluded the common carotid artery ( CCA ) or PPA to determine whether cerebral blood flow ( CBF ) values , infarct size and the stability of the model would be affected .
	manualset3
204675	7	417663	7	NULL	NULL	0	NULL	stability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While producing mouse MCAO models using commercially available silicone-coated monofilaments , we temporarily occluded the common carotid artery ( CCA ) or PPA to determine whether cerebral blood flow ( CBF ) values , infarct size and the stability of the model would be affected .
	manualset3
204676	8	417663	7	NULL	NULL	0	NULL	model	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	While producing mouse MCAO models using commercially available silicone-coated monofilaments , we temporarily occluded the common carotid artery ( CCA ) or PPA to determine whether cerebral blood flow ( CBF ) values , infarct size and the stability of the model would be affected .
	manualset3
204677	1	417664	7	NULL	NULL	0	NULL	 public opinion	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	While public opinion and reports from several police jurisdictions support the utility of juvenile curfews , recent empirical studies indicate that curfews are not effective at reducing juvenile offending or victimization .
	manualset3
204678	2	417664	7	NULL	NULL	0	NULL	reports	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	While public opinion and reports from several police jurisdictions support the utility of juvenile curfews , recent empirical studies indicate that curfews are not effective at reducing juvenile offending or victimization .
	manualset3
204679	3	417664	7	NULL	NULL	0	NULL	police jurisdictions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While public opinion and reports from several police jurisdictions support the utility of juvenile curfews , recent empirical studies indicate that curfews are not effective at reducing juvenile offending or victimization .
	manualset3
204680	4	417664	7	NULL	NULL	0	NULL	utility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While public opinion and reports from several police jurisdictions support the utility of juvenile curfews , recent empirical studies indicate that curfews are not effective at reducing juvenile offending or victimization .
	manualset3
204681	5	417664	7	NULL	NULL	0	NULL	juvenile curfews	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While public opinion and reports from several police jurisdictions support the utility of juvenile curfews , recent empirical studies indicate that curfews are not effective at reducing juvenile offending or victimization .
	manualset3
204682	6	417664	7	NULL	NULL	0	NULL	empirical studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While public opinion and reports from several police jurisdictions support the utility of juvenile curfews , recent empirical studies indicate that curfews are not effective at reducing juvenile offending or victimization .
	manualset3
204683	7	417664	7	NULL	NULL	0	NULL	curfews	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While public opinion and reports from several police jurisdictions support the utility of juvenile curfews , recent empirical studies indicate that curfews are not effective at reducing juvenile offending or victimization .
	manualset3
204684	8	417664	7	NULL	NULL	0	NULL	juvenile offending 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While public opinion and reports from several police jurisdictions support the utility of juvenile curfews , recent empirical studies indicate that curfews are not effective at reducing juvenile offending or victimization .
	manualset3
204685	9	417664	7	NULL	NULL	0	NULL	victimization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While public opinion and reports from several police jurisdictions support the utility of juvenile curfews , recent empirical studies indicate that curfews are not effective at reducing juvenile offending or victimization .
	manualset3
204686	1	417665	7	NULL	NULL	0	NULL	 rest EFCS	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While rest EFCS less than 40 % indicates poor LV functional reserve , good LV functional reserve is not always indicated by rest EFCS greater than or equal to 40 % .
	manualset3
204687	2	417665	7	NULL	NULL	0	NULL	 40 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While rest EFCS less than 40 % indicates poor LV functional reserve , good LV functional reserve is not always indicated by rest EFCS greater than or equal to 40 % .
	manualset3
204688	3	417665	7	NULL	NULL	0	NULL	LV functional reserve	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While rest EFCS less than 40 % indicates poor LV functional reserve , good LV functional reserve is not always indicated by rest EFCS greater than or equal to 40 % .
	manualset3
204689	4	417665	7	NULL	NULL	0	NULL	good LV functional reserve	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While rest EFCS less than 40 % indicates poor LV functional reserve , good LV functional reserve is not always indicated by rest EFCS greater than or equal to 40 % .
	manualset3
204690	5	417665	7	NULL	NULL	0	NULL	rest EFCS	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While rest EFCS less than 40 % indicates poor LV functional reserve , good LV functional reserve is not always indicated by rest EFCS greater than or equal to 40 % .
	manualset3
204691	6	417665	7	NULL	NULL	0	NULL	40 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While rest EFCS less than 40 % indicates poor LV functional reserve , good LV functional reserve is not always indicated by rest EFCS greater than or equal to 40 % .
	manualset3
204692	1	417666	7	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While risk of sensitisation to house dust mites generally increases with higher levels of exposure , this does not seem to hold for cats , where higher levels of cat allergen exposure are associated with less sensitisation .
	manualset3
204693	2	417666	7	NULL	NULL	NULL	NULL	sensitisation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While risk of sensitisation to house dust mites generally increases with higher levels of exposure , this does not seem to hold for cats , where higher levels of cat allergen exposure are associated with less sensitisation .
	manualset3
204694	3	417666	7	NULL	NULL	0	NULL	 house dust mites	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	While risk of sensitisation to house dust mites generally increases with higher levels of exposure , this does not seem to hold for cats , where higher levels of cat allergen exposure are associated with less sensitisation .
	manualset3
204695	4	417666	7	NULL	NULL	0	NULL	higher levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While risk of sensitisation to house dust mites generally increases with higher levels of exposure , this does not seem to hold for cats , where higher levels of cat allergen exposure are associated with less sensitisation .
	manualset3
204696	5	417666	7	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While risk of sensitisation to house dust mites generally increases with higher levels of exposure , this does not seem to hold for cats , where higher levels of cat allergen exposure are associated with less sensitisation .
	manualset3
204697	6	417666	7	NULL	NULL	0	NULL	cats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	While risk of sensitisation to house dust mites generally increases with higher levels of exposure , this does not seem to hold for cats , where higher levels of cat allergen exposure are associated with less sensitisation .
	manualset3
204698	7	417666	7	NULL	NULL	0	NULL	higher levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While risk of sensitisation to house dust mites generally increases with higher levels of exposure , this does not seem to hold for cats , where higher levels of cat allergen exposure are associated with less sensitisation .
	manualset3
204699	8	417666	7	NULL	NULL	0	NULL	cat allergen exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While risk of sensitisation to house dust mites generally increases with higher levels of exposure , this does not seem to hold for cats , where higher levels of cat allergen exposure are associated with less sensitisation .
	manualset3
204700	9	417666	7	NULL	NULL	NULL	NULL	less sensitisation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While risk of sensitisation to house dust mites generally increases with higher levels of exposure , this does not seem to hold for cats , where higher levels of cat allergen exposure are associated with less sensitisation .
	manualset3
204701	1	417667	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While some evidence was obtained suggesting a role of GABA in the motor effects of benzodiazepines , no evidence could be found for a role of GABA in their effects on sexual behavior .
	manualset3
204702	2	417667	7	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While some evidence was obtained suggesting a role of GABA in the motor effects of benzodiazepines , no evidence could be found for a role of GABA in their effects on sexual behavior .
	manualset3
204703	3	417667	7	NULL	NULL	0	NULL	GABA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While some evidence was obtained suggesting a role of GABA in the motor effects of benzodiazepines , no evidence could be found for a role of GABA in their effects on sexual behavior .
	manualset3
204704	4	417667	7	NULL	NULL	0	NULL	motor effects 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While some evidence was obtained suggesting a role of GABA in the motor effects of benzodiazepines , no evidence could be found for a role of GABA in their effects on sexual behavior .
	manualset3
204705	5	417667	7	NULL	NULL	0	NULL	benzodiazepines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While some evidence was obtained suggesting a role of GABA in the motor effects of benzodiazepines , no evidence could be found for a role of GABA in their effects on sexual behavior .
	manualset3
204706	6	417667	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While some evidence was obtained suggesting a role of GABA in the motor effects of benzodiazepines , no evidence could be found for a role of GABA in their effects on sexual behavior .
	manualset3
204707	7	417667	7	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While some evidence was obtained suggesting a role of GABA in the motor effects of benzodiazepines , no evidence could be found for a role of GABA in their effects on sexual behavior .
	manualset3
204708	8	417667	7	NULL	NULL	0	NULL	GABA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While some evidence was obtained suggesting a role of GABA in the motor effects of benzodiazepines , no evidence could be found for a role of GABA in their effects on sexual behavior .
	manualset3
204709	9	417667	7	NULL	NULL	NULL	NULL	effects	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While some evidence was obtained suggesting a role of GABA in the motor effects of benzodiazepines , no evidence could be found for a role of GABA in their effects on sexual behavior .
	manualset3
204710	10	417667	7	NULL	NULL	0	NULL	sexual behavior	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While some evidence was obtained suggesting a role of GABA in the motor effects of benzodiazepines , no evidence could be found for a role of GABA in their effects on sexual behavior .
	manualset3
204711	1	417668	7	NULL	NULL	NULL	NULL	trials	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While such trials will always remain the ` gold standard ' for establishing efficacy , they are unwieldy and inefficient for the rapid translation of our accelerating understanding of the molecular basis of cancer into preventive strategies .
	manualset3
204712	2	417668	7	NULL	NULL	0	NULL	` gold standard '	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While such trials will always remain the ` gold standard ' for establishing efficacy , they are unwieldy and inefficient for the rapid translation of our accelerating understanding of the molecular basis of cancer into preventive strategies .
	manualset3
204713	3	417668	7	NULL	NULL	0	NULL	rapid translation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While such trials will always remain the ` gold standard ' for establishing efficacy , they are unwieldy and inefficient for the rapid translation of our accelerating understanding of the molecular basis of cancer into preventive strategies .
	manualset3
204714	4	417668	7	NULL	NULL	0	NULL	accelerating understanding 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While such trials will always remain the ` gold standard ' for establishing efficacy , they are unwieldy and inefficient for the rapid translation of our accelerating understanding of the molecular basis of cancer into preventive strategies .
	manualset3
204715	5	417668	7	NULL	NULL	0	NULL	molecular basis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While such trials will always remain the ` gold standard ' for establishing efficacy , they are unwieldy and inefficient for the rapid translation of our accelerating understanding of the molecular basis of cancer into preventive strategies .
	manualset3
204716	6	417668	7	NULL	NULL	0	NULL	cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	While such trials will always remain the ` gold standard ' for establishing efficacy , they are unwieldy and inefficient for the rapid translation of our accelerating understanding of the molecular basis of cancer into preventive strategies .
	manualset3
204717	7	417668	7	NULL	NULL	NULL	NULL	preventive strategies	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While such trials will always remain the ` gold standard ' for establishing efficacy , they are unwieldy and inefficient for the rapid translation of our accelerating understanding of the molecular basis of cancer into preventive strategies .
	manualset3
204718	1	417669	7	NULL	NULL	0	NULL	 rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While such a rate is generally regarded as quite high , it is actually somewhat lower than one might expect based on the rate at which viral diversity could be generated within a single animal .
	manualset3
204719	2	417669	7	NULL	NULL	0	NULL	 rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While such a rate is generally regarded as quite high , it is actually somewhat lower than one might expect based on the rate at which viral diversity could be generated within a single animal .
	manualset3
204720	3	417669	7	NULL	NULL	0	NULL	viral diversity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While such a rate is generally regarded as quite high , it is actually somewhat lower than one might expect based on the rate at which viral diversity could be generated within a single animal .
	manualset3
204721	4	417669	7	NULL	NULL	0	NULL	single animal	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	While such a rate is generally regarded as quite high , it is actually somewhat lower than one might expect based on the rate at which viral diversity could be generated within a single animal .
	manualset3
204722	1	417670	7	NULL	NULL	0	NULL	N-terminal sequence	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	While the N-terminal sequence of the heavy chain , VELTQPGSMVLKPGQSLTI , showed similarity to the variable regions of those of teleost fishes Igs , the N-terminal sequence of the light chain , DIVLTQSPAVQSVQLGDT , was similar to the variable regions of chondrostei and mammalian kappa chains .
	manualset3
204723	2	417670	7	NULL	NULL	0	NULL	heavy chain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	While the N-terminal sequence of the heavy chain , VELTQPGSMVLKPGQSLTI , showed similarity to the variable regions of those of teleost fishes Igs , the N-terminal sequence of the light chain , DIVLTQSPAVQSVQLGDT , was similar to the variable regions of chondrostei and mammalian kappa chains .
	manualset3
204724	3	417670	7	NULL	NULL	0	NULL	VELTQPGSMVLKPGQSLTI	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	While the N-terminal sequence of the heavy chain , VELTQPGSMVLKPGQSLTI , showed similarity to the variable regions of those of teleost fishes Igs , the N-terminal sequence of the light chain , DIVLTQSPAVQSVQLGDT , was similar to the variable regions of chondrostei and mammalian kappa chains .
	manualset3
204725	4	417670	7	NULL	NULL	0	NULL	similarity	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	While the N-terminal sequence of the heavy chain , VELTQPGSMVLKPGQSLTI , showed similarity to the variable regions of those of teleost fishes Igs , the N-terminal sequence of the light chain , DIVLTQSPAVQSVQLGDT , was similar to the variable regions of chondrostei and mammalian kappa chains .
	manualset3
204726	5	417670	7	NULL	NULL	0	NULL	variable regions	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	While the N-terminal sequence of the heavy chain , VELTQPGSMVLKPGQSLTI , showed similarity to the variable regions of those of teleost fishes Igs , the N-terminal sequence of the light chain , DIVLTQSPAVQSVQLGDT , was similar to the variable regions of chondrostei and mammalian kappa chains .
	manualset3
204727	6	417670	7	NULL	NULL	0	NULL	teleost fishes Igs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	While the N-terminal sequence of the heavy chain , VELTQPGSMVLKPGQSLTI , showed similarity to the variable regions of those of teleost fishes Igs , the N-terminal sequence of the light chain , DIVLTQSPAVQSVQLGDT , was similar to the variable regions of chondrostei and mammalian kappa chains .
	manualset3
204728	7	417670	7	NULL	NULL	0	NULL	 N-terminal sequence	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	While the N-terminal sequence of the heavy chain , VELTQPGSMVLKPGQSLTI , showed similarity to the variable regions of those of teleost fishes Igs , the N-terminal sequence of the light chain , DIVLTQSPAVQSVQLGDT , was similar to the variable regions of chondrostei and mammalian kappa chains .
	manualset3
204729	8	417670	7	NULL	NULL	0	NULL	light chain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	While the N-terminal sequence of the heavy chain , VELTQPGSMVLKPGQSLTI , showed similarity to the variable regions of those of teleost fishes Igs , the N-terminal sequence of the light chain , DIVLTQSPAVQSVQLGDT , was similar to the variable regions of chondrostei and mammalian kappa chains .
	manualset3
204730	9	417670	7	NULL	NULL	0	NULL	DIVLTQSPAVQSVQLGDT	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	While the N-terminal sequence of the heavy chain , VELTQPGSMVLKPGQSLTI , showed similarity to the variable regions of those of teleost fishes Igs , the N-terminal sequence of the light chain , DIVLTQSPAVQSVQLGDT , was similar to the variable regions of chondrostei and mammalian kappa chains .
	manualset3
204731	10	417670	7	NULL	NULL	0	NULL	variable regions	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	While the N-terminal sequence of the heavy chain , VELTQPGSMVLKPGQSLTI , showed similarity to the variable regions of those of teleost fishes Igs , the N-terminal sequence of the light chain , DIVLTQSPAVQSVQLGDT , was similar to the variable regions of chondrostei and mammalian kappa chains .
	manualset3
204732	11	417670	7	NULL	NULL	0	NULL	chondrostei kappa chains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	While the N-terminal sequence of the heavy chain , VELTQPGSMVLKPGQSLTI , showed similarity to the variable regions of those of teleost fishes Igs , the N-terminal sequence of the light chain , DIVLTQSPAVQSVQLGDT , was similar to the variable regions of chondrostei and mammalian kappa chains .
	manualset3
204733	12	417670	7	NULL	NULL	0	NULL	mammalian kappa chains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	While the N-terminal sequence of the heavy chain , VELTQPGSMVLKPGQSLTI , showed similarity to the variable regions of those of teleost fishes Igs , the N-terminal sequence of the light chain , DIVLTQSPAVQSVQLGDT , was similar to the variable regions of chondrostei and mammalian kappa chains .
	manualset3
204734	1	417671	7	NULL	NULL	0	NULL	 bone	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	While the added bone produced by acetabular augmentation was durable , histological and biochemical analyses suggested that it had not undergone cartilage metaplasia .
	manualset3
204735	2	417671	7	NULL	NULL	0	NULL	acetabular augmentation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While the added bone produced by acetabular augmentation was durable , histological and biochemical analyses suggested that it had not undergone cartilage metaplasia .
	manualset3
204736	3	417671	7	NULL	NULL	0	NULL	histological analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While the added bone produced by acetabular augmentation was durable , histological and biochemical analyses suggested that it had not undergone cartilage metaplasia .
	manualset3
204737	4	417671	7	NULL	NULL	0	NULL	biochemical analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While the added bone produced by acetabular augmentation was durable , histological and biochemical analyses suggested that it had not undergone cartilage metaplasia .
	manualset3
204738	5	417671	7	NULL	NULL	0	NULL	cartilage metaplasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While the added bone produced by acetabular augmentation was durable , histological and biochemical analyses suggested that it had not undergone cartilage metaplasia .
	manualset3
204739	1	417672	7	NULL	NULL	NULL	NULL	expressions	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While the expressions of CD20 , CD33 , CD117 , HLA-DR were seen in some MM patients , the positive rates were 12.1 % , 15.2 % , 30.3 % , 9.1 % , respectively ; the expression of other antigens was negative .
	manualset3
204740	2	417672	7	NULL	NULL	0	NULL	CD20	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	While the expressions of CD20 , CD33 , CD117 , HLA-DR were seen in some MM patients , the positive rates were 12.1 % , 15.2 % , 30.3 % , 9.1 % , respectively ; the expression of other antigens was negative .
	manualset3
204741	3	417672	7	NULL	NULL	0	NULL	CD33	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	While the expressions of CD20 , CD33 , CD117 , HLA-DR were seen in some MM patients , the positive rates were 12.1 % , 15.2 % , 30.3 % , 9.1 % , respectively ; the expression of other antigens was negative .
	manualset3
204742	4	417672	7	NULL	NULL	0	NULL	CD117	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	While the expressions of CD20 , CD33 , CD117 , HLA-DR were seen in some MM patients , the positive rates were 12.1 % , 15.2 % , 30.3 % , 9.1 % , respectively ; the expression of other antigens was negative .
	manualset3
204743	5	417672	7	NULL	NULL	0	NULL	HLA-DR	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	While the expressions of CD20 , CD33 , CD117 , HLA-DR were seen in some MM patients , the positive rates were 12.1 % , 15.2 % , 30.3 % , 9.1 % , respectively ; the expression of other antigens was negative .
	manualset3
204744	6	417672	7	NULL	NULL	0	NULL	MM patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	While the expressions of CD20 , CD33 , CD117 , HLA-DR were seen in some MM patients , the positive rates were 12.1 % , 15.2 % , 30.3 % , 9.1 % , respectively ; the expression of other antigens was negative .
	manualset3
204745	7	417672	7	NULL	NULL	0	NULL	positive rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While the expressions of CD20 , CD33 , CD117 , HLA-DR were seen in some MM patients , the positive rates were 12.1 % , 15.2 % , 30.3 % , 9.1 % , respectively ; the expression of other antigens was negative .
	manualset3
204746	8	417672	7	NULL	NULL	0	NULL	12.1 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While the expressions of CD20 , CD33 , CD117 , HLA-DR were seen in some MM patients , the positive rates were 12.1 % , 15.2 % , 30.3 % , 9.1 % , respectively ; the expression of other antigens was negative .
	manualset3
204747	9	417672	7	NULL	NULL	0	NULL	15.2 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While the expressions of CD20 , CD33 , CD117 , HLA-DR were seen in some MM patients , the positive rates were 12.1 % , 15.2 % , 30.3 % , 9.1 % , respectively ; the expression of other antigens was negative .
	manualset3
204748	10	417672	7	NULL	NULL	0	NULL	30.3 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While the expressions of CD20 , CD33 , CD117 , HLA-DR were seen in some MM patients , the positive rates were 12.1 % , 15.2 % , 30.3 % , 9.1 % , respectively ; the expression of other antigens was negative .
	manualset3
204749	11	417672	7	NULL	NULL	0	NULL	9.1 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While the expressions of CD20 , CD33 , CD117 , HLA-DR were seen in some MM patients , the positive rates were 12.1 % , 15.2 % , 30.3 % , 9.1 % , respectively ; the expression of other antigens was negative .
	manualset3
204750	12	417672	7	NULL	NULL	0	NULL	expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While the expressions of CD20 , CD33 , CD117 , HLA-DR were seen in some MM patients , the positive rates were 12.1 % , 15.2 % , 30.3 % , 9.1 % , respectively ; the expression of other antigens was negative .
	manualset3
204751	13	417672	7	NULL	NULL	0	NULL	antigens	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	While the expressions of CD20 , CD33 , CD117 , HLA-DR were seen in some MM patients , the positive rates were 12.1 % , 15.2 % , 30.3 % , 9.1 % , respectively ; the expression of other antigens was negative .
	manualset3
204752	1	417673	7	NULL	NULL	0	NULL	 implantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	While the implantation of a central venous catheter is technically tiresome and subject to a complication rate up to 5 % , the peripheral venous cannulization , in general , does not represent any technical problem .
	manualset3
204753	2	417673	7	NULL	NULL	0	NULL	central venous catheter	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	While the implantation of a central venous catheter is technically tiresome and subject to a complication rate up to 5 % , the peripheral venous cannulization , in general , does not represent any technical problem .
	manualset3
204754	3	417673	7	NULL	NULL	NULL	NULL	complication rate	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While the implantation of a central venous catheter is technically tiresome and subject to a complication rate up to 5 % , the peripheral venous cannulization , in general , does not represent any technical problem .
	manualset3
204755	4	417673	7	NULL	NULL	0	NULL	5 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While the implantation of a central venous catheter is technically tiresome and subject to a complication rate up to 5 % , the peripheral venous cannulization , in general , does not represent any technical problem .
	manualset3
204756	5	417673	7	NULL	NULL	0	NULL	peripheral venous cannulization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	While the implantation of a central venous catheter is technically tiresome and subject to a complication rate up to 5 % , the peripheral venous cannulization , in general , does not represent any technical problem .
	manualset3
204757	6	417673	7	NULL	NULL	0	NULL	technical problem	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While the implantation of a central venous catheter is technically tiresome and subject to a complication rate up to 5 % , the peripheral venous cannulization , in general , does not represent any technical problem .
	manualset3
204758	1	417674	7	NULL	NULL	0	NULL	initial application	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	While the initial application of rituximab to patients with MS was based on the concept that B cell depletion may translate into decreases in potentially pathogenic CNS-autoreactive antibodies , insights from these studies have underscored the importance of non-antibody mediated functions of B cells .
	manualset3
204759	2	417674	7	NULL	NULL	0	NULL	 rituximab	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	While the initial application of rituximab to patients with MS was based on the concept that B cell depletion may translate into decreases in potentially pathogenic CNS-autoreactive antibodies , insights from these studies have underscored the importance of non-antibody mediated functions of B cells .
	manualset3
204760	3	417674	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	While the initial application of rituximab to patients with MS was based on the concept that B cell depletion may translate into decreases in potentially pathogenic CNS-autoreactive antibodies , insights from these studies have underscored the importance of non-antibody mediated functions of B cells .
	manualset3
204761	4	417674	7	NULL	NULL	0	NULL	MS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	While the initial application of rituximab to patients with MS was based on the concept that B cell depletion may translate into decreases in potentially pathogenic CNS-autoreactive antibodies , insights from these studies have underscored the importance of non-antibody mediated functions of B cells .
	manualset3
204762	5	417674	7	NULL	NULL	0	NULL	concept	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	While the initial application of rituximab to patients with MS was based on the concept that B cell depletion may translate into decreases in potentially pathogenic CNS-autoreactive antibodies , insights from these studies have underscored the importance of non-antibody mediated functions of B cells .
	manualset3
204763	6	417674	7	NULL	NULL	0	NULL	B cell depletion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While the initial application of rituximab to patients with MS was based on the concept that B cell depletion may translate into decreases in potentially pathogenic CNS-autoreactive antibodies , insights from these studies have underscored the importance of non-antibody mediated functions of B cells .
	manualset3
204764	7	417674	7	NULL	NULL	0	NULL	pathogenic CNS-autoreactive antibodies 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	While the initial application of rituximab to patients with MS was based on the concept that B cell depletion may translate into decreases in potentially pathogenic CNS-autoreactive antibodies , insights from these studies have underscored the importance of non-antibody mediated functions of B cells .
	manualset3
204765	8	417674	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While the initial application of rituximab to patients with MS was based on the concept that B cell depletion may translate into decreases in potentially pathogenic CNS-autoreactive antibodies , insights from these studies have underscored the importance of non-antibody mediated functions of B cells .
	manualset3
204766	9	417674	7	NULL	NULL	0	NULL	non-antibody mediated functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While the initial application of rituximab to patients with MS was based on the concept that B cell depletion may translate into decreases in potentially pathogenic CNS-autoreactive antibodies , insights from these studies have underscored the importance of non-antibody mediated functions of B cells .
	manualset3
204767	10	417674	7	NULL	NULL	0	NULL	B cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	While the initial application of rituximab to patients with MS was based on the concept that B cell depletion may translate into decreases in potentially pathogenic CNS-autoreactive antibodies , insights from these studies have underscored the importance of non-antibody mediated functions of B cells .
	manualset3
204768	1	417675	7	NULL	NULL	0	NULL	 introduction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While the introduction of 3 - ( 3 , 4 , 5-trimethoxyphenyl ) propanoic moiety resulted in a definite drop in potency and efficacy , esterification with 3 - ( 3 , 4 , 5-trimethoxyphenyl ) propiolic acid gave four isomers ( 3a-d ) that maintain high potency and possess optimal efficacy .
	manualset3
204769	2	417675	7	NULL	NULL	0	NULL	3 - ( 3 , 4 , 5-trimethoxyphenyl ) propanoic moiety	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While the introduction of 3 - ( 3 , 4 , 5-trimethoxyphenyl ) propanoic moiety resulted in a definite drop in potency and efficacy , esterification with 3 - ( 3 , 4 , 5-trimethoxyphenyl ) propiolic acid gave four isomers ( 3a-d ) that maintain high potency and possess optimal efficacy .
	manualset3
204770	3	417675	7	NULL	NULL	0	NULL	 drop	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While the introduction of 3 - ( 3 , 4 , 5-trimethoxyphenyl ) propanoic moiety resulted in a definite drop in potency and efficacy , esterification with 3 - ( 3 , 4 , 5-trimethoxyphenyl ) propiolic acid gave four isomers ( 3a-d ) that maintain high potency and possess optimal efficacy .
	manualset3
204771	4	417675	7	NULL	NULL	0	NULL	esterification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While the introduction of 3 - ( 3 , 4 , 5-trimethoxyphenyl ) propanoic moiety resulted in a definite drop in potency and efficacy , esterification with 3 - ( 3 , 4 , 5-trimethoxyphenyl ) propiolic acid gave four isomers ( 3a-d ) that maintain high potency and possess optimal efficacy .
	manualset3
204772	5	417675	7	NULL	NULL	0	NULL	3 - ( 3 , 4 , 5-trimethoxyphenyl ) propiolic acid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While the introduction of 3 - ( 3 , 4 , 5-trimethoxyphenyl ) propanoic moiety resulted in a definite drop in potency and efficacy , esterification with 3 - ( 3 , 4 , 5-trimethoxyphenyl ) propiolic acid gave four isomers ( 3a-d ) that maintain high potency and possess optimal efficacy .
	manualset3
204773	6	417675	7	NULL	NULL	NULL	NULL	 four isomers ( 3a-d )	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While the introduction of 3 - ( 3 , 4 , 5-trimethoxyphenyl ) propanoic moiety resulted in a definite drop in potency and efficacy , esterification with 3 - ( 3 , 4 , 5-trimethoxyphenyl ) propiolic acid gave four isomers ( 3a-d ) that maintain high potency and possess optimal efficacy .
	manualset3
204774	7	417675	7	NULL	NULL	0	NULL	high potency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While the introduction of 3 - ( 3 , 4 , 5-trimethoxyphenyl ) propanoic moiety resulted in a definite drop in potency and efficacy , esterification with 3 - ( 3 , 4 , 5-trimethoxyphenyl ) propiolic acid gave four isomers ( 3a-d ) that maintain high potency and possess optimal efficacy .
	manualset3
204775	8	417675	7	NULL	NULL	0	NULL	optimal efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While the introduction of 3 - ( 3 , 4 , 5-trimethoxyphenyl ) propanoic moiety resulted in a definite drop in potency and efficacy , esterification with 3 - ( 3 , 4 , 5-trimethoxyphenyl ) propiolic acid gave four isomers ( 3a-d ) that maintain high potency and possess optimal efficacy .
	manualset3
204776	9	417675	7	NULL	NULL	0	NULL	potency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While the introduction of 3 - ( 3 , 4 , 5-trimethoxyphenyl ) propanoic moiety resulted in a definite drop in potency and efficacy , esterification with 3 - ( 3 , 4 , 5-trimethoxyphenyl ) propiolic acid gave four isomers ( 3a-d ) that maintain high potency and possess optimal efficacy .
	manualset3
204777	10	417675	7	NULL	NULL	0	NULL	efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While the introduction of 3 - ( 3 , 4 , 5-trimethoxyphenyl ) propanoic moiety resulted in a definite drop in potency and efficacy , esterification with 3 - ( 3 , 4 , 5-trimethoxyphenyl ) propiolic acid gave four isomers ( 3a-d ) that maintain high potency and possess optimal efficacy .
	manualset3
204778	1	417676	7	NULL	NULL	0	NULL	medical device GMPs	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	While the medical device GMPs in the United States have been rewritten to accommodate a quality system approach similar to ISO 9000 , the Center for Biologics Evaluation and Research of the FDA is also beginning to make moves toward adopting `` quality systems audits '' as an inspection process rather than using the historical approach of record reviews .
	manualset3
204779	2	417676	7	NULL	NULL	0	NULL	United States	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	While the medical device GMPs in the United States have been rewritten to accommodate a quality system approach similar to ISO 9000 , the Center for Biologics Evaluation and Research of the FDA is also beginning to make moves toward adopting `` quality systems audits '' as an inspection process rather than using the historical approach of record reviews .
	manualset3
204780	3	417676	7	NULL	NULL	0	NULL	quality system approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While the medical device GMPs in the United States have been rewritten to accommodate a quality system approach similar to ISO 9000 , the Center for Biologics Evaluation and Research of the FDA is also beginning to make moves toward adopting `` quality systems audits '' as an inspection process rather than using the historical approach of record reviews .
	manualset3
204781	4	417676	7	NULL	NULL	0	NULL	ISO 9000	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While the medical device GMPs in the United States have been rewritten to accommodate a quality system approach similar to ISO 9000 , the Center for Biologics Evaluation and Research of the FDA is also beginning to make moves toward adopting `` quality systems audits '' as an inspection process rather than using the historical approach of record reviews .
	manualset3
204782	5	417676	7	NULL	NULL	0	NULL	Center for Biologics Evaluation and Research 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	While the medical device GMPs in the United States have been rewritten to accommodate a quality system approach similar to ISO 9000 , the Center for Biologics Evaluation and Research of the FDA is also beginning to make moves toward adopting `` quality systems audits '' as an inspection process rather than using the historical approach of record reviews .
	manualset3
204783	6	417676	7	NULL	NULL	0	NULL	FDA	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	While the medical device GMPs in the United States have been rewritten to accommodate a quality system approach similar to ISO 9000 , the Center for Biologics Evaluation and Research of the FDA is also beginning to make moves toward adopting `` quality systems audits '' as an inspection process rather than using the historical approach of record reviews .
	manualset3
204784	7	417676	7	NULL	NULL	0	NULL	quality systems audits	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While the medical device GMPs in the United States have been rewritten to accommodate a quality system approach similar to ISO 9000 , the Center for Biologics Evaluation and Research of the FDA is also beginning to make moves toward adopting `` quality systems audits '' as an inspection process rather than using the historical approach of record reviews .
	manualset3
204785	8	417676	7	NULL	NULL	0	NULL	inspection process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While the medical device GMPs in the United States have been rewritten to accommodate a quality system approach similar to ISO 9000 , the Center for Biologics Evaluation and Research of the FDA is also beginning to make moves toward adopting `` quality systems audits '' as an inspection process rather than using the historical approach of record reviews .
	manualset3
204786	9	417676	7	NULL	NULL	0	NULL	historical approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While the medical device GMPs in the United States have been rewritten to accommodate a quality system approach similar to ISO 9000 , the Center for Biologics Evaluation and Research of the FDA is also beginning to make moves toward adopting `` quality systems audits '' as an inspection process rather than using the historical approach of record reviews .
	manualset3
204787	10	417676	7	NULL	NULL	0	NULL	record reviews	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	While the medical device GMPs in the United States have been rewritten to accommodate a quality system approach similar to ISO 9000 , the Center for Biologics Evaluation and Research of the FDA is also beginning to make moves toward adopting `` quality systems audits '' as an inspection process rather than using the historical approach of record reviews .
	manualset3
204788	1	417677	7	NULL	NULL	0	NULL	modes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While the modes comprising the boson peak appear to be largely delocalized , there is a sharp drop in the participation ratio of the modes that exist just below the boson peak indicative of the quasilocalized nature of the low-frequency vibrations .
	manualset3
204789	2	417677	7	NULL	NULL	0	NULL	boson peak 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	While the modes comprising the boson peak appear to be largely delocalized , there is a sharp drop in the participation ratio of the modes that exist just below the boson peak indicative of the quasilocalized nature of the low-frequency vibrations .
	manualset3
204790	3	417677	7	NULL	NULL	0	NULL	sharp drop	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While the modes comprising the boson peak appear to be largely delocalized , there is a sharp drop in the participation ratio of the modes that exist just below the boson peak indicative of the quasilocalized nature of the low-frequency vibrations .
	manualset3
204791	4	417677	7	NULL	NULL	0	NULL	participation ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While the modes comprising the boson peak appear to be largely delocalized , there is a sharp drop in the participation ratio of the modes that exist just below the boson peak indicative of the quasilocalized nature of the low-frequency vibrations .
	manualset3
204792	5	417677	7	NULL	NULL	0	NULL	modes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While the modes comprising the boson peak appear to be largely delocalized , there is a sharp drop in the participation ratio of the modes that exist just below the boson peak indicative of the quasilocalized nature of the low-frequency vibrations .
	manualset3
204793	6	417677	7	NULL	NULL	0	NULL	boson peak	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	While the modes comprising the boson peak appear to be largely delocalized , there is a sharp drop in the participation ratio of the modes that exist just below the boson peak indicative of the quasilocalized nature of the low-frequency vibrations .
	manualset3
204794	7	417677	7	NULL	NULL	0	NULL	quasilocalized nature	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While the modes comprising the boson peak appear to be largely delocalized , there is a sharp drop in the participation ratio of the modes that exist just below the boson peak indicative of the quasilocalized nature of the low-frequency vibrations .
	manualset3
204795	8	417677	7	NULL	NULL	0	NULL	 low-frequency vibrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While the modes comprising the boson peak appear to be largely delocalized , there is a sharp drop in the participation ratio of the modes that exist just below the boson peak indicative of the quasilocalized nature of the low-frequency vibrations .
	manualset3
204796	1	417678	7	NULL	NULL	0	NULL	occurence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While the occurence of the MEN 2 syndrome is associated with mutations in the RET protooncogene , the reason for carcinogenesis in sMTC still remains unclear .
	manualset3
204797	2	417678	7	NULL	NULL	0	NULL	MEN 2 syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	While the occurence of the MEN 2 syndrome is associated with mutations in the RET protooncogene , the reason for carcinogenesis in sMTC still remains unclear .
	manualset3
204798	3	417678	7	NULL	NULL	0	NULL	mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While the occurence of the MEN 2 syndrome is associated with mutations in the RET protooncogene , the reason for carcinogenesis in sMTC still remains unclear .
	manualset3
204799	4	417678	7	NULL	NULL	0	NULL	RET protooncogene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	While the occurence of the MEN 2 syndrome is associated with mutations in the RET protooncogene , the reason for carcinogenesis in sMTC still remains unclear .
	manualset3
204800	5	417678	7	NULL	NULL	0	NULL	reason	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While the occurence of the MEN 2 syndrome is associated with mutations in the RET protooncogene , the reason for carcinogenesis in sMTC still remains unclear .
	manualset3
204801	6	417678	7	NULL	NULL	NULL	NULL	carcinogenesis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While the occurence of the MEN 2 syndrome is associated with mutations in the RET protooncogene , the reason for carcinogenesis in sMTC still remains unclear .
	manualset3
204802	7	417678	7	NULL	NULL	0	NULL	sMTC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	While the occurence of the MEN 2 syndrome is associated with mutations in the RET protooncogene , the reason for carcinogenesis in sMTC still remains unclear .
	manualset3
204803	1	417679	7	NULL	NULL	0	NULL	 parent cell line CV-1	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	While the parent cell line CV-1 only showed a weak spontaneous activation of the alternative pathway , Cl-4 cells additionally triggered the classical pathway of complement activation independent of anti-HIV antibodies by direct C1q binding .
	manualset3
204804	2	417679	7	NULL	NULL	0	NULL	weak spontaneous activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While the parent cell line CV-1 only showed a weak spontaneous activation of the alternative pathway , Cl-4 cells additionally triggered the classical pathway of complement activation independent of anti-HIV antibodies by direct C1q binding .
	manualset3
204805	3	417679	7	NULL	NULL	0	NULL	alternative pathway	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While the parent cell line CV-1 only showed a weak spontaneous activation of the alternative pathway , Cl-4 cells additionally triggered the classical pathway of complement activation independent of anti-HIV antibodies by direct C1q binding .
	manualset3
204806	4	417679	7	NULL	NULL	0	NULL	Cl-4 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	While the parent cell line CV-1 only showed a weak spontaneous activation of the alternative pathway , Cl-4 cells additionally triggered the classical pathway of complement activation independent of anti-HIV antibodies by direct C1q binding .
	manualset3
204807	5	417679	7	NULL	NULL	0	NULL	classical pathway	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While the parent cell line CV-1 only showed a weak spontaneous activation of the alternative pathway , Cl-4 cells additionally triggered the classical pathway of complement activation independent of anti-HIV antibodies by direct C1q binding .
	manualset3
204808	6	417679	7	NULL	NULL	0	NULL	complement activation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While the parent cell line CV-1 only showed a weak spontaneous activation of the alternative pathway , Cl-4 cells additionally triggered the classical pathway of complement activation independent of anti-HIV antibodies by direct C1q binding .
	manualset3
204809	7	417679	7	NULL	NULL	0	NULL	anti-HIV antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	While the parent cell line CV-1 only showed a weak spontaneous activation of the alternative pathway , Cl-4 cells additionally triggered the classical pathway of complement activation independent of anti-HIV antibodies by direct C1q binding .
	manualset3
204810	8	417679	7	NULL	NULL	0	NULL	direct C1q binding	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While the parent cell line CV-1 only showed a weak spontaneous activation of the alternative pathway , Cl-4 cells additionally triggered the classical pathway of complement activation independent of anti-HIV antibodies by direct C1q binding .
	manualset3
204811	1	417680	7	NULL	NULL	0	NULL	preparations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	While the preparations of influenza vaccines and a partially purified fraction of ribosomal vaccine from Pseudomonas aeruginosa exhibit a gelation of lysate with high levels of endotoxin , rubeola vaccines , interferon and a purified fraction of ribosomal vaccine , presented a negligible amount of endotoxin .
	manualset3
204812	2	417680	7	NULL	NULL	0	NULL	influenza vaccines	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	While the preparations of influenza vaccines and a partially purified fraction of ribosomal vaccine from Pseudomonas aeruginosa exhibit a gelation of lysate with high levels of endotoxin , rubeola vaccines , interferon and a purified fraction of ribosomal vaccine , presented a negligible amount of endotoxin .
	manualset3
204813	3	417680	7	NULL	NULL	0	NULL	partially purified fraction	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	While the preparations of influenza vaccines and a partially purified fraction of ribosomal vaccine from Pseudomonas aeruginosa exhibit a gelation of lysate with high levels of endotoxin , rubeola vaccines , interferon and a purified fraction of ribosomal vaccine , presented a negligible amount of endotoxin .
	manualset3
204814	4	417680	7	NULL	NULL	0	NULL	ribosomal vaccine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	While the preparations of influenza vaccines and a partially purified fraction of ribosomal vaccine from Pseudomonas aeruginosa exhibit a gelation of lysate with high levels of endotoxin , rubeola vaccines , interferon and a purified fraction of ribosomal vaccine , presented a negligible amount of endotoxin .
	manualset3
204815	5	417680	7	NULL	NULL	0	NULL	Pseudomonas aeruginosa	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	While the preparations of influenza vaccines and a partially purified fraction of ribosomal vaccine from Pseudomonas aeruginosa exhibit a gelation of lysate with high levels of endotoxin , rubeola vaccines , interferon and a purified fraction of ribosomal vaccine , presented a negligible amount of endotoxin .
	manualset3
204816	6	417680	7	NULL	NULL	0	NULL	gelation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While the preparations of influenza vaccines and a partially purified fraction of ribosomal vaccine from Pseudomonas aeruginosa exhibit a gelation of lysate with high levels of endotoxin , rubeola vaccines , interferon and a purified fraction of ribosomal vaccine , presented a negligible amount of endotoxin .
	manualset3
204817	7	417680	7	NULL	NULL	0	NULL	lysate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While the preparations of influenza vaccines and a partially purified fraction of ribosomal vaccine from Pseudomonas aeruginosa exhibit a gelation of lysate with high levels of endotoxin , rubeola vaccines , interferon and a purified fraction of ribosomal vaccine , presented a negligible amount of endotoxin .
	manualset3
204818	8	417680	7	NULL	NULL	0	NULL	high levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While the preparations of influenza vaccines and a partially purified fraction of ribosomal vaccine from Pseudomonas aeruginosa exhibit a gelation of lysate with high levels of endotoxin , rubeola vaccines , interferon and a purified fraction of ribosomal vaccine , presented a negligible amount of endotoxin .
	manualset3
204819	9	417680	7	NULL	NULL	0	NULL	endotoxin	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	While the preparations of influenza vaccines and a partially purified fraction of ribosomal vaccine from Pseudomonas aeruginosa exhibit a gelation of lysate with high levels of endotoxin , rubeola vaccines , interferon and a purified fraction of ribosomal vaccine , presented a negligible amount of endotoxin .
	manualset3
204820	10	417680	7	NULL	NULL	0	NULL	rubeola vaccines	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	While the preparations of influenza vaccines and a partially purified fraction of ribosomal vaccine from Pseudomonas aeruginosa exhibit a gelation of lysate with high levels of endotoxin , rubeola vaccines , interferon and a purified fraction of ribosomal vaccine , presented a negligible amount of endotoxin .
	manualset3
204821	11	417680	7	NULL	NULL	0	NULL	 interferon	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	While the preparations of influenza vaccines and a partially purified fraction of ribosomal vaccine from Pseudomonas aeruginosa exhibit a gelation of lysate with high levels of endotoxin , rubeola vaccines , interferon and a purified fraction of ribosomal vaccine , presented a negligible amount of endotoxin .
	manualset3
204822	12	417680	7	NULL	NULL	0	NULL	 purified fraction	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	While the preparations of influenza vaccines and a partially purified fraction of ribosomal vaccine from Pseudomonas aeruginosa exhibit a gelation of lysate with high levels of endotoxin , rubeola vaccines , interferon and a purified fraction of ribosomal vaccine , presented a negligible amount of endotoxin .
	manualset3
204823	13	417680	7	NULL	NULL	0	NULL	ribosomal vaccine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	While the preparations of influenza vaccines and a partially purified fraction of ribosomal vaccine from Pseudomonas aeruginosa exhibit a gelation of lysate with high levels of endotoxin , rubeola vaccines , interferon and a purified fraction of ribosomal vaccine , presented a negligible amount of endotoxin .
	manualset3
204824	14	417680	7	NULL	NULL	0	NULL	 negligible amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While the preparations of influenza vaccines and a partially purified fraction of ribosomal vaccine from Pseudomonas aeruginosa exhibit a gelation of lysate with high levels of endotoxin , rubeola vaccines , interferon and a purified fraction of ribosomal vaccine , presented a negligible amount of endotoxin .
	manualset3
204825	15	417680	7	NULL	NULL	0	NULL	 endotoxin	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	While the preparations of influenza vaccines and a partially purified fraction of ribosomal vaccine from Pseudomonas aeruginosa exhibit a gelation of lysate with high levels of endotoxin , rubeola vaccines , interferon and a purified fraction of ribosomal vaccine , presented a negligible amount of endotoxin .
	manualset3
204899	1	417681	7	NULL	NULL	0	NULL	species-endogenous level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While the species-endogenous level of rat heart IF1 ( i.e. , 1x IF1 ) inhibited IF1-depleted rat heart SMP virtually not at all at any ( KCl ) examined , the 8x rat heart IF1 was nearly as inhibitory as the 1x rabbit heart IF1 at varying ionic strengths .
	manualset3
204900	2	417681	7	NULL	NULL	NULL	NULL	rat heart IF1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While the species-endogenous level of rat heart IF1 ( i.e. , 1x IF1 ) inhibited IF1-depleted rat heart SMP virtually not at all at any ( KCl ) examined , the 8x rat heart IF1 was nearly as inhibitory as the 1x rabbit heart IF1 at varying ionic strengths .
	manualset3
204901	3	417681	7	NULL	NULL	0	NULL	1x IF1	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While the species-endogenous level of rat heart IF1 ( i.e. , 1x IF1 ) inhibited IF1-depleted rat heart SMP virtually not at all at any ( KCl ) examined , the 8x rat heart IF1 was nearly as inhibitory as the 1x rabbit heart IF1 at varying ionic strengths .
	manualset3
204902	4	417681	7	NULL	NULL	NULL	NULL	IF1-depleted rat heart SMP	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While the species-endogenous level of rat heart IF1 ( i.e. , 1x IF1 ) inhibited IF1-depleted rat heart SMP virtually not at all at any ( KCl ) examined , the 8x rat heart IF1 was nearly as inhibitory as the 1x rabbit heart IF1 at varying ionic strengths .
	manualset3
204903	5	417681	7	NULL	NULL	0	NULL	KCl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While the species-endogenous level of rat heart IF1 ( i.e. , 1x IF1 ) inhibited IF1-depleted rat heart SMP virtually not at all at any ( KCl ) examined , the 8x rat heart IF1 was nearly as inhibitory as the 1x rabbit heart IF1 at varying ionic strengths .
	manualset3
204904	6	417681	7	NULL	NULL	NULL	NULL	 8x rat heart IF1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While the species-endogenous level of rat heart IF1 ( i.e. , 1x IF1 ) inhibited IF1-depleted rat heart SMP virtually not at all at any ( KCl ) examined , the 8x rat heart IF1 was nearly as inhibitory as the 1x rabbit heart IF1 at varying ionic strengths .
	manualset3
204911	7	417681	7	NULL	NULL	0	NULL	1x rabbit heart IF1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	While the species-endogenous level of rat heart IF1 ( i.e. , 1x IF1 ) inhibited IF1-depleted rat heart SMP virtually not at all at any ( KCl ) examined , the 8x rat heart IF1 was nearly as inhibitory as the 1x rabbit heart IF1 at varying ionic strengths .
	manualset3
204914	8	417681	7	NULL	NULL	0	NULL	ionic strengths	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While the species-endogenous level of rat heart IF1 ( i.e. , 1x IF1 ) inhibited IF1-depleted rat heart SMP virtually not at all at any ( KCl ) examined , the 8x rat heart IF1 was nearly as inhibitory as the 1x rabbit heart IF1 at varying ionic strengths .
	manualset3
204917	1	417682	7	NULL	NULL	0	NULL	tissue distribution	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	While the tissue distribution of their products was found to be identical to that in mammals , the pattern of isoform expression is less complex .
	manualset3
204918	2	417682	7	NULL	NULL	0	NULL	products	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	While the tissue distribution of their products was found to be identical to that in mammals , the pattern of isoform expression is less complex .
	manualset3
204919	3	417682	7	NULL	NULL	0	NULL	mammals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	While the tissue distribution of their products was found to be identical to that in mammals , the pattern of isoform expression is less complex .
	manualset3
204920	4	417682	7	NULL	NULL	0	NULL	pattern	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While the tissue distribution of their products was found to be identical to that in mammals , the pattern of isoform expression is less complex .
	manualset3
204921	5	417682	7	NULL	NULL	0	NULL	isoform expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While the tissue distribution of their products was found to be identical to that in mammals , the pattern of isoform expression is less complex .
	manualset3
204923	1	417683	7	NULL	NULL	0	NULL	toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While the toxicity of hexavalent chromium is well established , trivalent chromium is an essential nutrient involved in insulin and glucose homeostasis .
	manualset3
204925	2	417683	7	NULL	NULL	0	NULL	hexavalent chromium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While the toxicity of hexavalent chromium is well established , trivalent chromium is an essential nutrient involved in insulin and glucose homeostasis .
	manualset3
204926	3	417683	7	NULL	NULL	0	NULL	 trivalent chromium 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While the toxicity of hexavalent chromium is well established , trivalent chromium is an essential nutrient involved in insulin and glucose homeostasis .
	manualset3
204927	4	417683	7	NULL	NULL	0	NULL	nutrient	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	While the toxicity of hexavalent chromium is well established , trivalent chromium is an essential nutrient involved in insulin and glucose homeostasis .
	manualset3
204928	5	417683	7	NULL	NULL	0	NULL	insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	While the toxicity of hexavalent chromium is well established , trivalent chromium is an essential nutrient involved in insulin and glucose homeostasis .
	manualset3
204929	6	417683	7	NULL	NULL	0	NULL	 glucose homeostasis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While the toxicity of hexavalent chromium is well established , trivalent chromium is an essential nutrient involved in insulin and glucose homeostasis .
	manualset3
204936	1	417684	7	NULL	NULL	0	NULL	variety	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While there are a variety of commercially available platforms for automated chromagen-based and fluorescence-based image acquisition of tissue microarrays , this chapter is focused on the analysis of fluorescent images by AQUA ( R ) analysis ( Automated QUantitative Analysis ) and the solutions offered by such a method for research and diagnostics .
	manualset3
204937	2	417684	7	NULL	NULL	0	NULL	commercially available platforms	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While there are a variety of commercially available platforms for automated chromagen-based and fluorescence-based image acquisition of tissue microarrays , this chapter is focused on the analysis of fluorescent images by AQUA ( R ) analysis ( Automated QUantitative Analysis ) and the solutions offered by such a method for research and diagnostics .
	manualset3
204942	3	417684	7	NULL	NULL	0	NULL	automated chromagen-based image acquisition	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While there are a variety of commercially available platforms for automated chromagen-based and fluorescence-based image acquisition of tissue microarrays , this chapter is focused on the analysis of fluorescent images by AQUA ( R ) analysis ( Automated QUantitative Analysis ) and the solutions offered by such a method for research and diagnostics .
	manualset3
204948	4	417684	7	NULL	NULL	0	NULL	fluorescence-based image acquisition	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While there are a variety of commercially available platforms for automated chromagen-based and fluorescence-based image acquisition of tissue microarrays , this chapter is focused on the analysis of fluorescent images by AQUA ( R ) analysis ( Automated QUantitative Analysis ) and the solutions offered by such a method for research and diagnostics .
	manualset3
204949	5	417684	7	NULL	NULL	0	NULL	tissue microarrays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While there are a variety of commercially available platforms for automated chromagen-based and fluorescence-based image acquisition of tissue microarrays , this chapter is focused on the analysis of fluorescent images by AQUA ( R ) analysis ( Automated QUantitative Analysis ) and the solutions offered by such a method for research and diagnostics .
	manualset3
204950	6	417684	7	NULL	NULL	0	NULL	chapter 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	While there are a variety of commercially available platforms for automated chromagen-based and fluorescence-based image acquisition of tissue microarrays , this chapter is focused on the analysis of fluorescent images by AQUA ( R ) analysis ( Automated QUantitative Analysis ) and the solutions offered by such a method for research and diagnostics .
	manualset3
204951	7	417684	7	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While there are a variety of commercially available platforms for automated chromagen-based and fluorescence-based image acquisition of tissue microarrays , this chapter is focused on the analysis of fluorescent images by AQUA ( R ) analysis ( Automated QUantitative Analysis ) and the solutions offered by such a method for research and diagnostics .
	manualset3
204952	8	417684	7	NULL	NULL	0	NULL	 fluorescent images	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While there are a variety of commercially available platforms for automated chromagen-based and fluorescence-based image acquisition of tissue microarrays , this chapter is focused on the analysis of fluorescent images by AQUA ( R ) analysis ( Automated QUantitative Analysis ) and the solutions offered by such a method for research and diagnostics .
	manualset3
204953	9	417684	7	NULL	NULL	0	NULL	AQUA ( R ) analysis ( Automated QUantitative Analysis )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While there are a variety of commercially available platforms for automated chromagen-based and fluorescence-based image acquisition of tissue microarrays , this chapter is focused on the analysis of fluorescent images by AQUA ( R ) analysis ( Automated QUantitative Analysis ) and the solutions offered by such a method for research and diagnostics .
	manualset3
204954	10	417684	7	NULL	NULL	0	NULL	solutions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While there are a variety of commercially available platforms for automated chromagen-based and fluorescence-based image acquisition of tissue microarrays , this chapter is focused on the analysis of fluorescent images by AQUA ( R ) analysis ( Automated QUantitative Analysis ) and the solutions offered by such a method for research and diagnostics .
	manualset3
204955	11	417684	7	NULL	NULL	0	NULL	 method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While there are a variety of commercially available platforms for automated chromagen-based and fluorescence-based image acquisition of tissue microarrays , this chapter is focused on the analysis of fluorescent images by AQUA ( R ) analysis ( Automated QUantitative Analysis ) and the solutions offered by such a method for research and diagnostics .
	manualset3
204956	12	417684	7	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While there are a variety of commercially available platforms for automated chromagen-based and fluorescence-based image acquisition of tissue microarrays , this chapter is focused on the analysis of fluorescent images by AQUA ( R ) analysis ( Automated QUantitative Analysis ) and the solutions offered by such a method for research and diagnostics .
	manualset3
204957	13	417684	7	NULL	NULL	0	NULL	diagnostics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While there are a variety of commercially available platforms for automated chromagen-based and fluorescence-based image acquisition of tissue microarrays , this chapter is focused on the analysis of fluorescent images by AQUA ( R ) analysis ( Automated QUantitative Analysis ) and the solutions offered by such a method for research and diagnostics .
	manualset3
204958	1	417685	7	NULL	NULL	0	NULL	speculation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While there has been a great deal of speculation over the years on the importance of emotional factors in inflammatory bowel disease ( IBD ) , it is only in the last decade or so that studies with stronger designs have been available to clarify the nature of this relationship .
	manualset3
204959	2	417685	7	NULL	NULL	0	NULL	years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	While there has been a great deal of speculation over the years on the importance of emotional factors in inflammatory bowel disease ( IBD ) , it is only in the last decade or so that studies with stronger designs have been available to clarify the nature of this relationship .
	manualset3
204960	3	417685	7	NULL	NULL	0	NULL	emotional factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	While there has been a great deal of speculation over the years on the importance of emotional factors in inflammatory bowel disease ( IBD ) , it is only in the last decade or so that studies with stronger designs have been available to clarify the nature of this relationship .
	manualset3
204961	4	417685	7	NULL	NULL	0	NULL	inflammatory bowel disease ( IBD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	While there has been a great deal of speculation over the years on the importance of emotional factors in inflammatory bowel disease ( IBD ) , it is only in the last decade or so that studies with stronger designs have been available to clarify the nature of this relationship .
	manualset3
204962	5	417685	7	NULL	NULL	0	NULL	 last decade	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	While there has been a great deal of speculation over the years on the importance of emotional factors in inflammatory bowel disease ( IBD ) , it is only in the last decade or so that studies with stronger designs have been available to clarify the nature of this relationship .
	manualset3
204963	6	417685	7	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While there has been a great deal of speculation over the years on the importance of emotional factors in inflammatory bowel disease ( IBD ) , it is only in the last decade or so that studies with stronger designs have been available to clarify the nature of this relationship .
	manualset3
204964	7	417685	7	NULL	NULL	0	NULL	stronger designs	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While there has been a great deal of speculation over the years on the importance of emotional factors in inflammatory bowel disease ( IBD ) , it is only in the last decade or so that studies with stronger designs have been available to clarify the nature of this relationship .
	manualset3
204965	8	417685	7	NULL	NULL	0	NULL	nature	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While there has been a great deal of speculation over the years on the importance of emotional factors in inflammatory bowel disease ( IBD ) , it is only in the last decade or so that studies with stronger designs have been available to clarify the nature of this relationship .
	manualset3
204966	9	417685	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	While there has been a great deal of speculation over the years on the importance of emotional factors in inflammatory bowel disease ( IBD ) , it is only in the last decade or so that studies with stronger designs have been available to clarify the nature of this relationship .
	manualset3
204967	10	417685	7	NULL	NULL	0	NULL	deal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While there has been a great deal of speculation over the years on the importance of emotional factors in inflammatory bowel disease ( IBD ) , it is only in the last decade or so that studies with stronger designs have been available to clarify the nature of this relationship .
	manualset3
204968	1	417686	7	NULL	NULL	0	NULL	current cure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While there is no current cure , recent work in the field of allogeneic hematopoietic stem cell transplantation ( HSCT ) and the induction of mixed chimerism , a state in which multilineage hematopoietic populations of both recipient and donor co-exist , has demonstrated that it is possible to provide protection from disease onset , as well as reverse the autoimmune state in spontaneously diabetic mice .
	manualset3
204969	2	417686	7	NULL	NULL	0	NULL	recent work	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While there is no current cure , recent work in the field of allogeneic hematopoietic stem cell transplantation ( HSCT ) and the induction of mixed chimerism , a state in which multilineage hematopoietic populations of both recipient and donor co-exist , has demonstrated that it is possible to provide protection from disease onset , as well as reverse the autoimmune state in spontaneously diabetic mice .
	manualset3
204970	3	417686	7	NULL	NULL	0	NULL	 field	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	While there is no current cure , recent work in the field of allogeneic hematopoietic stem cell transplantation ( HSCT ) and the induction of mixed chimerism , a state in which multilineage hematopoietic populations of both recipient and donor co-exist , has demonstrated that it is possible to provide protection from disease onset , as well as reverse the autoimmune state in spontaneously diabetic mice .
	manualset3
204971	4	417686	7	NULL	NULL	0	NULL	allogeneic hematopoietic stem cell transplantation ( HSCT ) 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	While there is no current cure , recent work in the field of allogeneic hematopoietic stem cell transplantation ( HSCT ) and the induction of mixed chimerism , a state in which multilineage hematopoietic populations of both recipient and donor co-exist , has demonstrated that it is possible to provide protection from disease onset , as well as reverse the autoimmune state in spontaneously diabetic mice .
	manualset3
204972	5	417686	7	NULL	NULL	0	NULL	 induction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While there is no current cure , recent work in the field of allogeneic hematopoietic stem cell transplantation ( HSCT ) and the induction of mixed chimerism , a state in which multilineage hematopoietic populations of both recipient and donor co-exist , has demonstrated that it is possible to provide protection from disease onset , as well as reverse the autoimmune state in spontaneously diabetic mice .
	manualset3
204973	6	417686	7	NULL	NULL	0	NULL	mixed chimerism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While there is no current cure , recent work in the field of allogeneic hematopoietic stem cell transplantation ( HSCT ) and the induction of mixed chimerism , a state in which multilineage hematopoietic populations of both recipient and donor co-exist , has demonstrated that it is possible to provide protection from disease onset , as well as reverse the autoimmune state in spontaneously diabetic mice .
	manualset3
204974	7	417686	7	NULL	NULL	NULL	NULL	state	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While there is no current cure , recent work in the field of allogeneic hematopoietic stem cell transplantation ( HSCT ) and the induction of mixed chimerism , a state in which multilineage hematopoietic populations of both recipient and donor co-exist , has demonstrated that it is possible to provide protection from disease onset , as well as reverse the autoimmune state in spontaneously diabetic mice .
	manualset3
204975	8	417686	7	NULL	NULL	0	NULL	multilineage hematopoietic populations	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	While there is no current cure , recent work in the field of allogeneic hematopoietic stem cell transplantation ( HSCT ) and the induction of mixed chimerism , a state in which multilineage hematopoietic populations of both recipient and donor co-exist , has demonstrated that it is possible to provide protection from disease onset , as well as reverse the autoimmune state in spontaneously diabetic mice .
	manualset3
204976	9	417686	7	NULL	NULL	0	NULL	recipient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	While there is no current cure , recent work in the field of allogeneic hematopoietic stem cell transplantation ( HSCT ) and the induction of mixed chimerism , a state in which multilineage hematopoietic populations of both recipient and donor co-exist , has demonstrated that it is possible to provide protection from disease onset , as well as reverse the autoimmune state in spontaneously diabetic mice .
	manualset3
204977	10	417686	7	NULL	NULL	0	NULL	donor	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	While there is no current cure , recent work in the field of allogeneic hematopoietic stem cell transplantation ( HSCT ) and the induction of mixed chimerism , a state in which multilineage hematopoietic populations of both recipient and donor co-exist , has demonstrated that it is possible to provide protection from disease onset , as well as reverse the autoimmune state in spontaneously diabetic mice .
	manualset3
204978	11	417686	7	NULL	NULL	0	NULL	protection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While there is no current cure , recent work in the field of allogeneic hematopoietic stem cell transplantation ( HSCT ) and the induction of mixed chimerism , a state in which multilineage hematopoietic populations of both recipient and donor co-exist , has demonstrated that it is possible to provide protection from disease onset , as well as reverse the autoimmune state in spontaneously diabetic mice .
	manualset3
204979	12	417686	7	NULL	NULL	0	NULL	disease onset	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While there is no current cure , recent work in the field of allogeneic hematopoietic stem cell transplantation ( HSCT ) and the induction of mixed chimerism , a state in which multilineage hematopoietic populations of both recipient and donor co-exist , has demonstrated that it is possible to provide protection from disease onset , as well as reverse the autoimmune state in spontaneously diabetic mice .
	manualset3
204980	13	417686	7	NULL	NULL	0	NULL	 reverse 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While there is no current cure , recent work in the field of allogeneic hematopoietic stem cell transplantation ( HSCT ) and the induction of mixed chimerism , a state in which multilineage hematopoietic populations of both recipient and donor co-exist , has demonstrated that it is possible to provide protection from disease onset , as well as reverse the autoimmune state in spontaneously diabetic mice .
	manualset3
204981	14	417686	7	NULL	NULL	0	NULL	autoimmune state	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While there is no current cure , recent work in the field of allogeneic hematopoietic stem cell transplantation ( HSCT ) and the induction of mixed chimerism , a state in which multilineage hematopoietic populations of both recipient and donor co-exist , has demonstrated that it is possible to provide protection from disease onset , as well as reverse the autoimmune state in spontaneously diabetic mice .
	manualset3
204982	15	417686	7	NULL	NULL	0	NULL	diabetic mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	While there is no current cure , recent work in the field of allogeneic hematopoietic stem cell transplantation ( HSCT ) and the induction of mixed chimerism , a state in which multilineage hematopoietic populations of both recipient and donor co-exist , has demonstrated that it is possible to provide protection from disease onset , as well as reverse the autoimmune state in spontaneously diabetic mice .
	manualset3
205048	1	417687	7	NULL	NULL	0	NULL	perfect solution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While there is no perfect solution to merging the differing conventions , it is important that those performing and teaching bedside US and echo have a thorough understanding of the issues involved , and adopt a consistent approach .
	manualset3
205049	2	417687	7	NULL	NULL	0	NULL	conventions	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While there is no perfect solution to merging the differing conventions , it is important that those performing and teaching bedside US and echo have a thorough understanding of the issues involved , and adopt a consistent approach .
	manualset3
205056	3	417687	7	NULL	NULL	0	NULL	performing bedside US	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	While there is no perfect solution to merging the differing conventions , it is important that those performing and teaching bedside US and echo have a thorough understanding of the issues involved , and adopt a consistent approach .
	manualset3
205057	4	417687	7	NULL	NULL	0	NULL	teaching bedside US 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	While there is no perfect solution to merging the differing conventions , it is important that those performing and teaching bedside US and echo have a thorough understanding of the issues involved , and adopt a consistent approach .
	manualset3
205060	5	417687	7	NULL	NULL	0	NULL	performing bedside echo	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	While there is no perfect solution to merging the differing conventions , it is important that those performing and teaching bedside US and echo have a thorough understanding of the issues involved , and adopt a consistent approach .
	manualset3
205062	6	417687	7	NULL	NULL	0	NULL	teaching bedside echo	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	While there is no perfect solution to merging the differing conventions , it is important that those performing and teaching bedside US and echo have a thorough understanding of the issues involved , and adopt a consistent approach .
	manualset3
205065	7	417687	7	NULL	NULL	0	NULL	understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While there is no perfect solution to merging the differing conventions , it is important that those performing and teaching bedside US and echo have a thorough understanding of the issues involved , and adopt a consistent approach .
	manualset3
205068	8	417687	7	NULL	NULL	NULL	NULL	 issues 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While there is no perfect solution to merging the differing conventions , it is important that those performing and teaching bedside US and echo have a thorough understanding of the issues involved , and adopt a consistent approach .
	manualset3
205071	9	417687	7	NULL	NULL	0	NULL	consistent approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While there is no perfect solution to merging the differing conventions , it is important that those performing and teaching bedside US and echo have a thorough understanding of the issues involved , and adopt a consistent approach .
	manualset3
205073	1	417688	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While these results show that long-term adaptation ( LTA ) extends to 5-HT neuromodulation , no phenotype switch could be detected in the postsynaptic muscle .
	manualset3
205076	2	417688	7	NULL	NULL	0	NULL	 long-term adaptation ( LTA 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While these results show that long-term adaptation ( LTA ) extends to 5-HT neuromodulation , no phenotype switch could be detected in the postsynaptic muscle .
	manualset3
205077	3	417688	7	NULL	NULL	0	NULL	5-HT neuromodulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While these results show that long-term adaptation ( LTA ) extends to 5-HT neuromodulation , no phenotype switch could be detected in the postsynaptic muscle .
	manualset3
205080	4	417688	7	NULL	NULL	0	NULL	phenotype	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	While these results show that long-term adaptation ( LTA ) extends to 5-HT neuromodulation , no phenotype switch could be detected in the postsynaptic muscle .
	manualset3
205082	5	417688	7	NULL	NULL	0	NULL	postsynaptic muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	While these results show that long-term adaptation ( LTA ) extends to 5-HT neuromodulation , no phenotype switch could be detected in the postsynaptic muscle .
	manualset3
205086	1	417689	7	NULL	NULL	0	NULL	squamous cell cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	While this squamous cell cancer responds to chemotherapy , successful treatment of lymphatic metastases can only be achieved with aggressive surgical treatment in combination with chemotherapy .
	manualset3
205088	2	417689	7	NULL	NULL	0	NULL	chemotherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	While this squamous cell cancer responds to chemotherapy , successful treatment of lymphatic metastases can only be achieved with aggressive surgical treatment in combination with chemotherapy .
	manualset3
205089	3	417689	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	While this squamous cell cancer responds to chemotherapy , successful treatment of lymphatic metastases can only be achieved with aggressive surgical treatment in combination with chemotherapy .
	manualset3
205090	4	417689	7	NULL	NULL	0	NULL	 lymphatic metastases	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While this squamous cell cancer responds to chemotherapy , successful treatment of lymphatic metastases can only be achieved with aggressive surgical treatment in combination with chemotherapy .
	manualset3
205091	5	417689	7	NULL	NULL	0	NULL	aggressive surgical treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	While this squamous cell cancer responds to chemotherapy , successful treatment of lymphatic metastases can only be achieved with aggressive surgical treatment in combination with chemotherapy .
	manualset3
205092	6	417689	7	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While this squamous cell cancer responds to chemotherapy , successful treatment of lymphatic metastases can only be achieved with aggressive surgical treatment in combination with chemotherapy .
	manualset3
205093	7	417689	7	NULL	NULL	0	NULL	chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	While this squamous cell cancer responds to chemotherapy , successful treatment of lymphatic metastases can only be achieved with aggressive surgical treatment in combination with chemotherapy .
	manualset3
205094	1	417690	7	NULL	NULL	NULL	NULL	ultrasound measures	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While ultrasound measures of OE muscle function showed poor association with EMG ( r = 0.28 , p = 0.22 ) , TrA and OI function showed moderate to excellent association ( TrA : r = 0.74 , p & lt ; 0.000 ; OI : r = 0.85 , p & lt ; 0.000 ) .
	manualset3
205096	2	417690	7	NULL	NULL	0	NULL	OE muscle function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While ultrasound measures of OE muscle function showed poor association with EMG ( r = 0.28 , p = 0.22 ) , TrA and OI function showed moderate to excellent association ( TrA : r = 0.74 , p & lt ; 0.000 ; OI : r = 0.85 , p & lt ; 0.000 ) .
	manualset3
205097	3	417690	7	NULL	NULL	0	NULL	poor association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	While ultrasound measures of OE muscle function showed poor association with EMG ( r = 0.28 , p = 0.22 ) , TrA and OI function showed moderate to excellent association ( TrA : r = 0.74 , p & lt ; 0.000 ; OI : r = 0.85 , p & lt ; 0.000 ) .
	manualset3
205103	4	417690	7	NULL	NULL	0	NULL	EMG	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	While ultrasound measures of OE muscle function showed poor association with EMG ( r = 0.28 , p = 0.22 ) , TrA and OI function showed moderate to excellent association ( TrA : r = 0.74 , p & lt ; 0.000 ; OI : r = 0.85 , p & lt ; 0.000 ) .
	manualset3
205104	5	417690	7	NULL	NULL	0	NULL	 r = 0.28	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	While ultrasound measures of OE muscle function showed poor association with EMG ( r = 0.28 , p = 0.22 ) , TrA and OI function showed moderate to excellent association ( TrA : r = 0.74 , p & lt ; 0.000 ; OI : r = 0.85 , p & lt ; 0.000 ) .
	manualset3
205105	6	417690	7	NULL	NULL	0	NULL	p = 0.22	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	While ultrasound measures of OE muscle function showed poor association with EMG ( r = 0.28 , p = 0.22 ) , TrA and OI function showed moderate to excellent association ( TrA : r = 0.74 , p & lt ; 0.000 ; OI : r = 0.85 , p & lt ; 0.000 ) .
	manualset3
205106	7	417690	7	NULL	NULL	NULL	NULL	 TrA function	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While ultrasound measures of OE muscle function showed poor association with EMG ( r = 0.28 , p = 0.22 ) , TrA and OI function showed moderate to excellent association ( TrA : r = 0.74 , p & lt ; 0.000 ; OI : r = 0.85 , p & lt ; 0.000 ) .
	manualset3
205107	8	417690	7	NULL	NULL	NULL	NULL	OI function	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While ultrasound measures of OE muscle function showed poor association with EMG ( r = 0.28 , p = 0.22 ) , TrA and OI function showed moderate to excellent association ( TrA : r = 0.74 , p & lt ; 0.000 ; OI : r = 0.85 , p & lt ; 0.000 ) .
	manualset3
205108	9	417690	7	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	While ultrasound measures of OE muscle function showed poor association with EMG ( r = 0.28 , p = 0.22 ) , TrA and OI function showed moderate to excellent association ( TrA : r = 0.74 , p & lt ; 0.000 ; OI : r = 0.85 , p & lt ; 0.000 ) .
	manualset3
205109	10	417690	7	NULL	NULL	0	NULL	TrA	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	While ultrasound measures of OE muscle function showed poor association with EMG ( r = 0.28 , p = 0.22 ) , TrA and OI function showed moderate to excellent association ( TrA : r = 0.74 , p & lt ; 0.000 ; OI : r = 0.85 , p & lt ; 0.000 ) .
	manualset3
205110	11	417690	7	NULL	NULL	0	NULL	r = 0.74	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	While ultrasound measures of OE muscle function showed poor association with EMG ( r = 0.28 , p = 0.22 ) , TrA and OI function showed moderate to excellent association ( TrA : r = 0.74 , p & lt ; 0.000 ; OI : r = 0.85 , p & lt ; 0.000 ) .
	manualset3
205111	12	417690	7	NULL	NULL	NULL	NULL	p & lt; 0.000 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While ultrasound measures of OE muscle function showed poor association with EMG ( r = 0.28 , p = 0.22 ) , TrA and OI function showed moderate to excellent association ( TrA : r = 0.74 , p & lt ; 0.000 ; OI : r = 0.85 , p & lt ; 0.000 ) .
	manualset3
205113	14	417690	7	NULL	NULL	0	NULL	OI	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	While ultrasound measures of OE muscle function showed poor association with EMG ( r = 0.28 , p = 0.22 ) , TrA and OI function showed moderate to excellent association ( TrA : r = 0.74 , p & lt ; 0.000 ; OI : r = 0.85 , p & lt ; 0.000 ) .
	manualset3
205114	15	417690	7	NULL	NULL	0	NULL	r = 0.85	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	While ultrasound measures of OE muscle function showed poor association with EMG ( r = 0.28 , p = 0.22 ) , TrA and OI function showed moderate to excellent association ( TrA : r = 0.74 , p & lt ; 0.000 ; OI : r = 0.85 , p & lt ; 0.000 ) .
	manualset3
205115	16	417690	7	NULL	NULL	0	NULL	p & lt ; 0.000 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	While ultrasound measures of OE muscle function showed poor association with EMG ( r = 0.28 , p = 0.22 ) , TrA and OI function showed moderate to excellent association ( TrA : r = 0.74 , p & lt ; 0.000 ; OI : r = 0.85 , p & lt ; 0.000 ) .
	manualset3
205116	1	417691	7	NULL	NULL	0	NULL	unimodality analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While unimodality analyses showed widespread brain atrophy and hypoperfusion in the patients , jICA further revealed two significant joint components of variations between atrophy and hypoperfusion across brain regions .
	manualset3
205117	2	417691	7	NULL	NULL	NULL	NULL	brain atrophy 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While unimodality analyses showed widespread brain atrophy and hypoperfusion in the patients , jICA further revealed two significant joint components of variations between atrophy and hypoperfusion across brain regions .
	manualset3
205118	3	417691	7	NULL	NULL	0	NULL	hypoperfusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While unimodality analyses showed widespread brain atrophy and hypoperfusion in the patients , jICA further revealed two significant joint components of variations between atrophy and hypoperfusion across brain regions .
	manualset3
205119	4	417691	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	While unimodality analyses showed widespread brain atrophy and hypoperfusion in the patients , jICA further revealed two significant joint components of variations between atrophy and hypoperfusion across brain regions .
	manualset3
205120	5	417691	7	NULL	NULL	0	NULL	 jICA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While unimodality analyses showed widespread brain atrophy and hypoperfusion in the patients , jICA further revealed two significant joint components of variations between atrophy and hypoperfusion across brain regions .
	manualset3
205121	6	417691	7	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While unimodality analyses showed widespread brain atrophy and hypoperfusion in the patients , jICA further revealed two significant joint components of variations between atrophy and hypoperfusion across brain regions .
	manualset3
205122	7	417691	7	NULL	NULL	0	NULL	joint components	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While unimodality analyses showed widespread brain atrophy and hypoperfusion in the patients , jICA further revealed two significant joint components of variations between atrophy and hypoperfusion across brain regions .
	manualset3
205123	8	417691	7	NULL	NULL	0	NULL	variations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While unimodality analyses showed widespread brain atrophy and hypoperfusion in the patients , jICA further revealed two significant joint components of variations between atrophy and hypoperfusion across brain regions .
	manualset3
205124	9	417691	7	NULL	NULL	0	NULL	atrophy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While unimodality analyses showed widespread brain atrophy and hypoperfusion in the patients , jICA further revealed two significant joint components of variations between atrophy and hypoperfusion across brain regions .
	manualset3
205125	10	417691	7	NULL	NULL	0	NULL	hypoperfusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While unimodality analyses showed widespread brain atrophy and hypoperfusion in the patients , jICA further revealed two significant joint components of variations between atrophy and hypoperfusion across brain regions .
	manualset3
205126	11	417691	7	NULL	NULL	0	NULL	brain regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	While unimodality analyses showed widespread brain atrophy and hypoperfusion in the patients , jICA further revealed two significant joint components of variations between atrophy and hypoperfusion across brain regions .
	manualset3
205127	1	417692	7	NULL	NULL	0	NULL	primary cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	While use of primary cells or cell line models for differentiating or differentiated tissue is widespread , the ability to assess factor binding and histone modification in tissue defines the events that occur in vivo and provides corroboration for studies in cultured cells .
	manualset3
205128	2	417692	7	NULL	NULL	0	NULL	cell line models	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	While use of primary cells or cell line models for differentiating or differentiated tissue is widespread , the ability to assess factor binding and histone modification in tissue defines the events that occur in vivo and provides corroboration for studies in cultured cells .
	manualset3
205129	3	417692	7	NULL	NULL	0	NULL	differentiated tissue 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	While use of primary cells or cell line models for differentiating or differentiated tissue is widespread , the ability to assess factor binding and histone modification in tissue defines the events that occur in vivo and provides corroboration for studies in cultured cells .
	manualset3
205130	4	417692	7	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While use of primary cells or cell line models for differentiating or differentiated tissue is widespread , the ability to assess factor binding and histone modification in tissue defines the events that occur in vivo and provides corroboration for studies in cultured cells .
	manualset3
205131	5	417692	7	NULL	NULL	0	NULL	factor binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While use of primary cells or cell line models for differentiating or differentiated tissue is widespread , the ability to assess factor binding and histone modification in tissue defines the events that occur in vivo and provides corroboration for studies in cultured cells .
	manualset3
205132	6	417692	7	NULL	NULL	0	NULL	histone modification	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While use of primary cells or cell line models for differentiating or differentiated tissue is widespread , the ability to assess factor binding and histone modification in tissue defines the events that occur in vivo and provides corroboration for studies in cultured cells .
	manualset3
205133	7	417692	7	NULL	NULL	0	NULL	tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	While use of primary cells or cell line models for differentiating or differentiated tissue is widespread , the ability to assess factor binding and histone modification in tissue defines the events that occur in vivo and provides corroboration for studies in cultured cells .
	manualset3
205134	8	417692	7	NULL	NULL	0	NULL	events	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While use of primary cells or cell line models for differentiating or differentiated tissue is widespread , the ability to assess factor binding and histone modification in tissue defines the events that occur in vivo and provides corroboration for studies in cultured cells .
	manualset3
205135	9	417692	7	NULL	NULL	0	NULL	corroboration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While use of primary cells or cell line models for differentiating or differentiated tissue is widespread , the ability to assess factor binding and histone modification in tissue defines the events that occur in vivo and provides corroboration for studies in cultured cells .
	manualset3
205136	10	417692	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	While use of primary cells or cell line models for differentiating or differentiated tissue is widespread , the ability to assess factor binding and histone modification in tissue defines the events that occur in vivo and provides corroboration for studies in cultured cells .
	manualset3
205137	11	417692	7	NULL	NULL	0	NULL	cultured cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	While use of primary cells or cell line models for differentiating or differentiated tissue is widespread , the ability to assess factor binding and histone modification in tissue defines the events that occur in vivo and provides corroboration for studies in cultured cells .
	manualset3
205138	12	417692	7	NULL	NULL	0	NULL	differentiating tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	While use of primary cells or cell line models for differentiating or differentiated tissue is widespread , the ability to assess factor binding and histone modification in tissue defines the events that occur in vivo and provides corroboration for studies in cultured cells .
	manualset3
205139	1	417693	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients underwent a Tl-scintigraphy examination .
	manualset3
205140	2	417693	7	NULL	NULL	0	NULL	Tl-scintigraphy examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients underwent a Tl-scintigraphy examination .
	manualset3
205141	1	417694	7	NULL	NULL	0	NULL	cardiac injury 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While we focus on cardiac injury and responses of the left ventricle ( LV ) , the mechanisms reviewed here have pathways in common with other wound healing models .
	manualset3
205142	2	417694	7	NULL	NULL	0	NULL	responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While we focus on cardiac injury and responses of the left ventricle ( LV ) , the mechanisms reviewed here have pathways in common with other wound healing models .
	manualset3
205143	3	417694	7	NULL	NULL	0	NULL	 left ventricle ( LV ) 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	While we focus on cardiac injury and responses of the left ventricle ( LV ) , the mechanisms reviewed here have pathways in common with other wound healing models .
	manualset3
205144	4	417694	7	NULL	NULL	0	NULL	mechanisms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While we focus on cardiac injury and responses of the left ventricle ( LV ) , the mechanisms reviewed here have pathways in common with other wound healing models .
	manualset3
205145	5	417694	7	NULL	NULL	0	NULL	pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While we focus on cardiac injury and responses of the left ventricle ( LV ) , the mechanisms reviewed here have pathways in common with other wound healing models .
	manualset3
205146	6	417694	7	NULL	NULL	NULL	NULL	wound healing models	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While we focus on cardiac injury and responses of the left ventricle ( LV ) , the mechanisms reviewed here have pathways in common with other wound healing models .
	manualset3
205147	1	417695	7	NULL	NULL	0	NULL	adherence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While we know that better adherence can improve BP during several months , the magnitude of this relationship in the short term is poorly understood .
	manualset3
205148	2	417695	7	NULL	NULL	0	NULL	BP	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While we know that better adherence can improve BP during several months , the magnitude of this relationship in the short term is poorly understood .
	manualset3
205149	3	417695	7	NULL	NULL	0	NULL	several months	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	While we know that better adherence can improve BP during several months , the magnitude of this relationship in the short term is poorly understood .
	manualset3
205150	4	417695	7	NULL	NULL	0	NULL	magnitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While we know that better adherence can improve BP during several months , the magnitude of this relationship in the short term is poorly understood .
	manualset3
205151	5	417695	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	While we know that better adherence can improve BP during several months , the magnitude of this relationship in the short term is poorly understood .
	manualset3
205152	6	417695	7	NULL	NULL	0	NULL	short term	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	While we know that better adherence can improve BP during several months , the magnitude of this relationship in the short term is poorly understood .
	manualset3
205153	1	417696	7	NULL	NULL	0	NULL	MN-based vaccines 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Whilst MN-based vaccines have demonstrated proof-of-concept in mice , it is vital to understand how MN targeting of VLPs to the skin epidermis affects activation and migration of Langerhans cells ( LCs ) in the real human skin environment .
	manualset3
205154	2	417696	7	NULL	NULL	0	NULL	proof-of-concept	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Whilst MN-based vaccines have demonstrated proof-of-concept in mice , it is vital to understand how MN targeting of VLPs to the skin epidermis affects activation and migration of Langerhans cells ( LCs ) in the real human skin environment .
	manualset3
205155	3	417696	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Whilst MN-based vaccines have demonstrated proof-of-concept in mice , it is vital to understand how MN targeting of VLPs to the skin epidermis affects activation and migration of Langerhans cells ( LCs ) in the real human skin environment .
	manualset3
205156	4	417696	7	NULL	NULL	NULL	NULL	MN targeting	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Whilst MN-based vaccines have demonstrated proof-of-concept in mice , it is vital to understand how MN targeting of VLPs to the skin epidermis affects activation and migration of Langerhans cells ( LCs ) in the real human skin environment .
	manualset3
205157	5	417696	7	NULL	NULL	0	NULL	VLPs 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Whilst MN-based vaccines have demonstrated proof-of-concept in mice , it is vital to understand how MN targeting of VLPs to the skin epidermis affects activation and migration of Langerhans cells ( LCs ) in the real human skin environment .
	manualset3
205158	6	417696	7	NULL	NULL	0	NULL	skin epidermis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Whilst MN-based vaccines have demonstrated proof-of-concept in mice , it is vital to understand how MN targeting of VLPs to the skin epidermis affects activation and migration of Langerhans cells ( LCs ) in the real human skin environment .
	manualset3
205159	7	417696	7	NULL	NULL	0	NULL	activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Whilst MN-based vaccines have demonstrated proof-of-concept in mice , it is vital to understand how MN targeting of VLPs to the skin epidermis affects activation and migration of Langerhans cells ( LCs ) in the real human skin environment .
	manualset3
205160	8	417696	7	NULL	NULL	0	NULL	migration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Whilst MN-based vaccines have demonstrated proof-of-concept in mice , it is vital to understand how MN targeting of VLPs to the skin epidermis affects activation and migration of Langerhans cells ( LCs ) in the real human skin environment .
	manualset3
205161	9	417696	7	NULL	NULL	0	NULL	Langerhans cells ( LCs )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Whilst MN-based vaccines have demonstrated proof-of-concept in mice , it is vital to understand how MN targeting of VLPs to the skin epidermis affects activation and migration of Langerhans cells ( LCs ) in the real human skin environment .
	manualset3
205162	10	417696	7	NULL	NULL	0	NULL	real human skin environment	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Whilst MN-based vaccines have demonstrated proof-of-concept in mice , it is vital to understand how MN targeting of VLPs to the skin epidermis affects activation and migration of Langerhans cells ( LCs ) in the real human skin environment .
	manualset3
205163	1	417697	7	NULL	NULL	0	NULL	TSP	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Whilst TSP in pre-menopausal breast cancer was slightly lower than in post-menopausal breast cancer , it did not correlate with estrogen receptors ( ER ) or progesterone receptors ( PR ) , but was negatively correlated with tissue-type plasminogen activator ( tPA ) , an oestradiol-inducible enzyme .
	manualset3
205164	2	417697	7	NULL	NULL	0	NULL	pre-menopausal breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Whilst TSP in pre-menopausal breast cancer was slightly lower than in post-menopausal breast cancer , it did not correlate with estrogen receptors ( ER ) or progesterone receptors ( PR ) , but was negatively correlated with tissue-type plasminogen activator ( tPA ) , an oestradiol-inducible enzyme .
	manualset3
205165	3	417697	7	NULL	NULL	0	NULL	post-menopausal breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Whilst TSP in pre-menopausal breast cancer was slightly lower than in post-menopausal breast cancer , it did not correlate with estrogen receptors ( ER ) or progesterone receptors ( PR ) , but was negatively correlated with tissue-type plasminogen activator ( tPA ) , an oestradiol-inducible enzyme .
	manualset3
205166	4	417697	7	NULL	NULL	0	NULL	estrogen receptors ( ER )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Whilst TSP in pre-menopausal breast cancer was slightly lower than in post-menopausal breast cancer , it did not correlate with estrogen receptors ( ER ) or progesterone receptors ( PR ) , but was negatively correlated with tissue-type plasminogen activator ( tPA ) , an oestradiol-inducible enzyme .
	manualset3
205167	5	417697	7	NULL	NULL	0	NULL	progesterone receptors ( PR )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Whilst TSP in pre-menopausal breast cancer was slightly lower than in post-menopausal breast cancer , it did not correlate with estrogen receptors ( ER ) or progesterone receptors ( PR ) , but was negatively correlated with tissue-type plasminogen activator ( tPA ) , an oestradiol-inducible enzyme .
	manualset3
205168	6	417697	7	NULL	NULL	0	NULL	tissue-type plasminogen activator ( tPA )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Whilst TSP in pre-menopausal breast cancer was slightly lower than in post-menopausal breast cancer , it did not correlate with estrogen receptors ( ER ) or progesterone receptors ( PR ) , but was negatively correlated with tissue-type plasminogen activator ( tPA ) , an oestradiol-inducible enzyme .
	manualset3
205169	7	417697	7	NULL	NULL	0	NULL	oestradiol-inducible enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Whilst TSP in pre-menopausal breast cancer was slightly lower than in post-menopausal breast cancer , it did not correlate with estrogen receptors ( ER ) or progesterone receptors ( PR ) , but was negatively correlated with tissue-type plasminogen activator ( tPA ) , an oestradiol-inducible enzyme .
	manualset3
205170	1	417698	7	NULL	NULL	0	NULL	graft samples	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Whilst the different graft samples induced varying levels of cytokine secretion in vitro , no distinct pattern suggesting a non-trivial relationship was observed .
	manualset3
205171	2	417698	7	NULL	NULL	0	NULL	 varying levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Whilst the different graft samples induced varying levels of cytokine secretion in vitro , no distinct pattern suggesting a non-trivial relationship was observed .
	manualset3
205172	3	417698	7	NULL	NULL	0	NULL	cytokine secretion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Whilst the different graft samples induced varying levels of cytokine secretion in vitro , no distinct pattern suggesting a non-trivial relationship was observed .
	manualset3
205173	5	417698	7	NULL	NULL	NULL	NULL	 non-trivial relationship	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Whilst the different graft samples induced varying levels of cytokine secretion in vitro , no distinct pattern suggesting a non-trivial relationship was observed .
	manualset3
205174	4	417698	7	NULL	NULL	0	NULL	pattern	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Whilst the different graft samples induced varying levels of cytokine secretion in vitro , no distinct pattern suggesting a non-trivial relationship was observed .
	manualset3
205175	1	417699	7	NULL	NULL	0	NULL	Whites	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Whites have more black neighbors in metropolitan areas with high levels of government employment and ample new housing ; whites have fewer black neighbors in metropolitan areas with a high level of municipal fragmentation .
	manualset3
205176	2	417699	7	NULL	NULL	0	NULL	black neighbors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Whites have more black neighbors in metropolitan areas with high levels of government employment and ample new housing ; whites have fewer black neighbors in metropolitan areas with a high level of municipal fragmentation .
	manualset3
205177	3	417699	7	NULL	NULL	0	NULL	metropolitan areas	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Whites have more black neighbors in metropolitan areas with high levels of government employment and ample new housing ; whites have fewer black neighbors in metropolitan areas with a high level of municipal fragmentation .
	manualset3
205178	4	417699	7	NULL	NULL	0	NULL	high levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Whites have more black neighbors in metropolitan areas with high levels of government employment and ample new housing ; whites have fewer black neighbors in metropolitan areas with a high level of municipal fragmentation .
	manualset3
205179	5	417699	7	NULL	NULL	0	NULL	government employment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Whites have more black neighbors in metropolitan areas with high levels of government employment and ample new housing ; whites have fewer black neighbors in metropolitan areas with a high level of municipal fragmentation .
	manualset3
205180	6	417699	7	NULL	NULL	0	NULL	whites	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Whites have more black neighbors in metropolitan areas with high levels of government employment and ample new housing ; whites have fewer black neighbors in metropolitan areas with a high level of municipal fragmentation .
	manualset3
205181	7	417699	7	NULL	NULL	0	NULL	black neighbors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Whites have more black neighbors in metropolitan areas with high levels of government employment and ample new housing ; whites have fewer black neighbors in metropolitan areas with a high level of municipal fragmentation .
	manualset3
205182	8	417699	7	NULL	NULL	0	NULL	metropolitan areas	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Whites have more black neighbors in metropolitan areas with high levels of government employment and ample new housing ; whites have fewer black neighbors in metropolitan areas with a high level of municipal fragmentation .
	manualset3
205183	9	417699	7	NULL	NULL	0	NULL	high level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Whites have more black neighbors in metropolitan areas with high levels of government employment and ample new housing ; whites have fewer black neighbors in metropolitan areas with a high level of municipal fragmentation .
	manualset3
205184	10	417699	7	NULL	NULL	0	NULL	 municipal fragmentation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Whites have more black neighbors in metropolitan areas with high levels of government employment and ample new housing ; whites have fewer black neighbors in metropolitan areas with a high level of municipal fragmentation .
	manualset3
205185	1	417700	7	NULL	NULL	0	NULL	Whole-cell recordings	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole-cell recordings were made from neurons in the rostral nucleus of the solitary tract in horizontal brainstem slices .
	manualset3
205186	2	417700	7	NULL	NULL	0	NULL	neurons 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole-cell recordings were made from neurons in the rostral nucleus of the solitary tract in horizontal brainstem slices .
	manualset3
205187	3	417700	7	NULL	NULL	0	NULL	rostral nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole-cell recordings were made from neurons in the rostral nucleus of the solitary tract in horizontal brainstem slices .
	manualset3
205188	4	417700	7	NULL	NULL	0	NULL	solitary tract 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole-cell recordings were made from neurons in the rostral nucleus of the solitary tract in horizontal brainstem slices .
	manualset3
205189	5	417700	7	NULL	NULL	NULL	NULL	horizontal brainstem slices	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Whole-cell recordings were made from neurons in the rostral nucleus of the solitary tract in horizontal brainstem slices .
	manualset3
205190	1	417701	7	NULL	NULL	0	NULL	Whole-mount electron microscopic observations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole-mount electron microscopic observations of the chromosomes directly spread onto a water surface revealed a configuration in which the above-described regions were localized on a continuous DNA fiber .
	manualset3
205191	2	417701	7	NULL	NULL	0	NULL	chromosomes	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole-mount electron microscopic observations of the chromosomes directly spread onto a water surface revealed a configuration in which the above-described regions were localized on a continuous DNA fiber .
	manualset3
205192	3	417701	7	NULL	NULL	0	NULL	water surface	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole-mount electron microscopic observations of the chromosomes directly spread onto a water surface revealed a configuration in which the above-described regions were localized on a continuous DNA fiber .
	manualset3
205193	4	417701	7	NULL	NULL	0	NULL	configuration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole-mount electron microscopic observations of the chromosomes directly spread onto a water surface revealed a configuration in which the above-described regions were localized on a continuous DNA fiber .
	manualset3
205194	5	417701	7	NULL	NULL	0	NULL	above-described regions 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole-mount electron microscopic observations of the chromosomes directly spread onto a water surface revealed a configuration in which the above-described regions were localized on a continuous DNA fiber .
	manualset3
205195	6	417701	7	NULL	NULL	0	NULL	continuous DNA fiber	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole-mount electron microscopic observations of the chromosomes directly spread onto a water surface revealed a configuration in which the above-described regions were localized on a continuous DNA fiber .
	manualset3
205196	1	417702	7	NULL	NULL	0	NULL	cell recordings	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole cell recordings from slices obtained during daytime ( n = 40 ) revealed neurons with a mean membrane potential of -66 + / -1.2 mV , input conductance of 1.5 + / -0.1 nS and state-dependent tonic or burst firing patterns .
	manualset3
205197	2	417702	7	NULL	NULL	0	NULL	slices 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole cell recordings from slices obtained during daytime ( n = 40 ) revealed neurons with a mean membrane potential of -66 + / -1.2 mV , input conductance of 1.5 + / -0.1 nS and state-dependent tonic or burst firing patterns .
	manualset3
205198	3	417702	7	NULL	NULL	0	NULL	daytime	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole cell recordings from slices obtained during daytime ( n = 40 ) revealed neurons with a mean membrane potential of -66 + / -1.2 mV , input conductance of 1.5 + / -0.1 nS and state-dependent tonic or burst firing patterns .
	manualset3
205199	4	417702	7	NULL	NULL	0	NULL	n = 40	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole cell recordings from slices obtained during daytime ( n = 40 ) revealed neurons with a mean membrane potential of -66 + / -1.2 mV , input conductance of 1.5 + / -0.1 nS and state-dependent tonic or burst firing patterns .
	manualset3
205200	5	417702	7	NULL	NULL	0	NULL	neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole cell recordings from slices obtained during daytime ( n = 40 ) revealed neurons with a mean membrane potential of -66 + / -1.2 mV , input conductance of 1.5 + / -0.1 nS and state-dependent tonic or burst firing patterns .
	manualset3
205201	6	417702	7	NULL	NULL	0	NULL	mean membrane potential 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole cell recordings from slices obtained during daytime ( n = 40 ) revealed neurons with a mean membrane potential of -66 + / -1.2 mV , input conductance of 1.5 + / -0.1 nS and state-dependent tonic or burst firing patterns .
	manualset3
205202	7	417702	7	NULL	NULL	0	NULL	-66 + / -1.2 mV	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole cell recordings from slices obtained during daytime ( n = 40 ) revealed neurons with a mean membrane potential of -66 + / -1.2 mV , input conductance of 1.5 + / -0.1 nS and state-dependent tonic or burst firing patterns .
	manualset3
205203	8	417702	7	NULL	NULL	0	NULL	input conductance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole cell recordings from slices obtained during daytime ( n = 40 ) revealed neurons with a mean membrane potential of -66 + / -1.2 mV , input conductance of 1.5 + / -0.1 nS and state-dependent tonic or burst firing patterns .
	manualset3
205204	9	417702	7	NULL	NULL	0	NULL	1.5 + / -0.1 nS	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole cell recordings from slices obtained during daytime ( n = 40 ) revealed neurons with a mean membrane potential of -66 + / -1.2 mV , input conductance of 1.5 + / -0.1 nS and state-dependent tonic or burst firing patterns .
	manualset3
205205	10	417702	7	NULL	NULL	0	NULL	state-dependent tonic firing patterns	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole cell recordings from slices obtained during daytime ( n = 40 ) revealed neurons with a mean membrane potential of -66 + / -1.2 mV , input conductance of 1.5 + / -0.1 nS and state-dependent tonic or burst firing patterns .
	manualset3
205206	11	417702	7	NULL	NULL	0	NULL	 burst firing patterns	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole cell recordings from slices obtained during daytime ( n = 40 ) revealed neurons with a mean membrane potential of -66 + / -1.2 mV , input conductance of 1.5 + / -0.1 nS and state-dependent tonic or burst firing patterns .
	manualset3
205248	1	417703	7	NULL	NULL	NULL	NULL	Whole genome analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Whole genome analysis uncovers heterogeneous identity structures of the hexon and fiber genes amongst the HAdV-14 and the B1/B2 subspecies , which may be important in prescient vaccine development .
	manualset3
205253	2	417703	7	NULL	NULL	0	NULL	heterogeneous identity structures 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole genome analysis uncovers heterogeneous identity structures of the hexon and fiber genes amongst the HAdV-14 and the B1/B2 subspecies , which may be important in prescient vaccine development .
	manualset3
205256	3	417703	7	NULL	NULL	0	NULL	hexon and fiber genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole genome analysis uncovers heterogeneous identity structures of the hexon and fiber genes amongst the HAdV-14 and the B1/B2 subspecies , which may be important in prescient vaccine development .
	manualset3
205258	4	417703	7	NULL	NULL	0	NULL	HAdV-14 subspecies	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole genome analysis uncovers heterogeneous identity structures of the hexon and fiber genes amongst the HAdV-14 and the B1/B2 subspecies , which may be important in prescient vaccine development .
	manualset3
205259	5	417703	7	NULL	NULL	0	NULL	B1/B2 subspecies	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole genome analysis uncovers heterogeneous identity structures of the hexon and fiber genes amongst the HAdV-14 and the B1/B2 subspecies , which may be important in prescient vaccine development .
	manualset3
205260	6	417703	7	NULL	NULL	0	NULL	vaccine development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole genome analysis uncovers heterogeneous identity structures of the hexon and fiber genes amongst the HAdV-14 and the B1/B2 subspecies , which may be important in prescient vaccine development .
	manualset3
205261	1	417704	7	NULL	NULL	0	NULL	Whole mounts 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole mounts of rat and guinea pig myenteric preparations were dually labeled with antibodies against the CB ( 1 ) receptor and choline acetyltransferase , neurofilament proteins , calbindin , calretinin , synapsin I , microtubule-associated protein-2 , calcitonin gene-related peptide , or substance P. The pattern of CB ( 1 ) receptor labeling and the neurochemical classification of CB ( 1 ) receptor-positive cells were markedly influenced by the species and fixation procedure .
	manualset3
205262	2	417704	7	NULL	NULL	0	NULL	rat  myenteric preparations	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole mounts of rat and guinea pig myenteric preparations were dually labeled with antibodies against the CB ( 1 ) receptor and choline acetyltransferase , neurofilament proteins , calbindin , calretinin , synapsin I , microtubule-associated protein-2 , calcitonin gene-related peptide , or substance P. The pattern of CB ( 1 ) receptor labeling and the neurochemical classification of CB ( 1 ) receptor-positive cells were markedly influenced by the species and fixation procedure .
	manualset3
205263	3	417704	7	NULL	NULL	0	NULL	guinea pig myenteric preparations 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole mounts of rat and guinea pig myenteric preparations were dually labeled with antibodies against the CB ( 1 ) receptor and choline acetyltransferase , neurofilament proteins , calbindin , calretinin , synapsin I , microtubule-associated protein-2 , calcitonin gene-related peptide , or substance P. The pattern of CB ( 1 ) receptor labeling and the neurochemical classification of CB ( 1 ) receptor-positive cells were markedly influenced by the species and fixation procedure .
	manualset3
205265	4	417704	7	NULL	NULL	0	NULL	antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole mounts of rat and guinea pig myenteric preparations were dually labeled with antibodies against the CB ( 1 ) receptor and choline acetyltransferase , neurofilament proteins , calbindin , calretinin , synapsin I , microtubule-associated protein-2 , calcitonin gene-related peptide , or substance P. The pattern of CB ( 1 ) receptor labeling and the neurochemical classification of CB ( 1 ) receptor-positive cells were markedly influenced by the species and fixation procedure .
	manualset3
205266	5	417704	7	NULL	NULL	0	NULL	CB ( 1 ) receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole mounts of rat and guinea pig myenteric preparations were dually labeled with antibodies against the CB ( 1 ) receptor and choline acetyltransferase , neurofilament proteins , calbindin , calretinin , synapsin I , microtubule-associated protein-2 , calcitonin gene-related peptide , or substance P. The pattern of CB ( 1 ) receptor labeling and the neurochemical classification of CB ( 1 ) receptor-positive cells were markedly influenced by the species and fixation procedure .
	manualset3
205267	6	417704	7	NULL	NULL	0	NULL	choline acetyltransferase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole mounts of rat and guinea pig myenteric preparations were dually labeled with antibodies against the CB ( 1 ) receptor and choline acetyltransferase , neurofilament proteins , calbindin , calretinin , synapsin I , microtubule-associated protein-2 , calcitonin gene-related peptide , or substance P. The pattern of CB ( 1 ) receptor labeling and the neurochemical classification of CB ( 1 ) receptor-positive cells were markedly influenced by the species and fixation procedure .
	manualset3
205268	7	417704	7	NULL	NULL	0	NULL	neurofilament proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole mounts of rat and guinea pig myenteric preparations were dually labeled with antibodies against the CB ( 1 ) receptor and choline acetyltransferase , neurofilament proteins , calbindin , calretinin , synapsin I , microtubule-associated protein-2 , calcitonin gene-related peptide , or substance P. The pattern of CB ( 1 ) receptor labeling and the neurochemical classification of CB ( 1 ) receptor-positive cells were markedly influenced by the species and fixation procedure .
	manualset3
205269	8	417704	7	NULL	NULL	0	NULL	calbindin	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole mounts of rat and guinea pig myenteric preparations were dually labeled with antibodies against the CB ( 1 ) receptor and choline acetyltransferase , neurofilament proteins , calbindin , calretinin , synapsin I , microtubule-associated protein-2 , calcitonin gene-related peptide , or substance P. The pattern of CB ( 1 ) receptor labeling and the neurochemical classification of CB ( 1 ) receptor-positive cells were markedly influenced by the species and fixation procedure .
	manualset3
205270	9	417704	7	NULL	NULL	0	NULL	calretinin	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole mounts of rat and guinea pig myenteric preparations were dually labeled with antibodies against the CB ( 1 ) receptor and choline acetyltransferase , neurofilament proteins , calbindin , calretinin , synapsin I , microtubule-associated protein-2 , calcitonin gene-related peptide , or substance P. The pattern of CB ( 1 ) receptor labeling and the neurochemical classification of CB ( 1 ) receptor-positive cells were markedly influenced by the species and fixation procedure .
	manualset3
205273	10	417704	7	NULL	NULL	0	NULL	synapsin I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole mounts of rat and guinea pig myenteric preparations were dually labeled with antibodies against the CB ( 1 ) receptor and choline acetyltransferase , neurofilament proteins , calbindin , calretinin , synapsin I , microtubule-associated protein-2 , calcitonin gene-related peptide , or substance P. The pattern of CB ( 1 ) receptor labeling and the neurochemical classification of CB ( 1 ) receptor-positive cells were markedly influenced by the species and fixation procedure .
	manualset3
205276	11	417704	7	NULL	NULL	0	NULL	microtubule-associated protein-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole mounts of rat and guinea pig myenteric preparations were dually labeled with antibodies against the CB ( 1 ) receptor and choline acetyltransferase , neurofilament proteins , calbindin , calretinin , synapsin I , microtubule-associated protein-2 , calcitonin gene-related peptide , or substance P. The pattern of CB ( 1 ) receptor labeling and the neurochemical classification of CB ( 1 ) receptor-positive cells were markedly influenced by the species and fixation procedure .
	manualset3
205278	12	417704	7	NULL	NULL	0	NULL	calcitonin gene-related peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole mounts of rat and guinea pig myenteric preparations were dually labeled with antibodies against the CB ( 1 ) receptor and choline acetyltransferase , neurofilament proteins , calbindin , calretinin , synapsin I , microtubule-associated protein-2 , calcitonin gene-related peptide , or substance P. The pattern of CB ( 1 ) receptor labeling and the neurochemical classification of CB ( 1 ) receptor-positive cells were markedly influenced by the species and fixation procedure .
	manualset3
205282	13	417704	7	NULL	NULL	0	NULL	substance P	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole mounts of rat and guinea pig myenteric preparations were dually labeled with antibodies against the CB ( 1 ) receptor and choline acetyltransferase , neurofilament proteins , calbindin , calretinin , synapsin I , microtubule-associated protein-2 , calcitonin gene-related peptide , or substance P. The pattern of CB ( 1 ) receptor labeling and the neurochemical classification of CB ( 1 ) receptor-positive cells were markedly influenced by the species and fixation procedure .
	manualset3
205283	14	417704	7	NULL	NULL	0	NULL	pattern 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole mounts of rat and guinea pig myenteric preparations were dually labeled with antibodies against the CB ( 1 ) receptor and choline acetyltransferase , neurofilament proteins , calbindin , calretinin , synapsin I , microtubule-associated protein-2 , calcitonin gene-related peptide , or substance P. The pattern of CB ( 1 ) receptor labeling and the neurochemical classification of CB ( 1 ) receptor-positive cells were markedly influenced by the species and fixation procedure .
	manualset3
205284	15	417704	7	NULL	NULL	0	NULL	CB ( 1 ) receptor labeling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole mounts of rat and guinea pig myenteric preparations were dually labeled with antibodies against the CB ( 1 ) receptor and choline acetyltransferase , neurofilament proteins , calbindin , calretinin , synapsin I , microtubule-associated protein-2 , calcitonin gene-related peptide , or substance P. The pattern of CB ( 1 ) receptor labeling and the neurochemical classification of CB ( 1 ) receptor-positive cells were markedly influenced by the species and fixation procedure .
	manualset3
205286	16	417704	7	NULL	NULL	0	NULL	neurochemical classification	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole mounts of rat and guinea pig myenteric preparations were dually labeled with antibodies against the CB ( 1 ) receptor and choline acetyltransferase , neurofilament proteins , calbindin , calretinin , synapsin I , microtubule-associated protein-2 , calcitonin gene-related peptide , or substance P. The pattern of CB ( 1 ) receptor labeling and the neurochemical classification of CB ( 1 ) receptor-positive cells were markedly influenced by the species and fixation procedure .
	manualset3
205287	17	417704	7	NULL	NULL	0	NULL	CB ( 1 ) receptor-positive cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole mounts of rat and guinea pig myenteric preparations were dually labeled with antibodies against the CB ( 1 ) receptor and choline acetyltransferase , neurofilament proteins , calbindin , calretinin , synapsin I , microtubule-associated protein-2 , calcitonin gene-related peptide , or substance P. The pattern of CB ( 1 ) receptor labeling and the neurochemical classification of CB ( 1 ) receptor-positive cells were markedly influenced by the species and fixation procedure .
	manualset3
205292	18	417704	7	NULL	NULL	0	NULL	species and fixation procedure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Whole mounts of rat and guinea pig myenteric preparations were dually labeled with antibodies against the CB ( 1 ) receptor and choline acetyltransferase , neurofilament proteins , calbindin , calretinin , synapsin I , microtubule-associated protein-2 , calcitonin gene-related peptide , or substance P. The pattern of CB ( 1 ) receptor labeling and the neurochemical classification of CB ( 1 ) receptor-positive cells were markedly influenced by the species and fixation procedure .
	manualset3
205294	1	417705	7	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients underwent nephroureterectomy and the four got well but one died of acute heart failure .
	manualset3
205295	2	417705	7	NULL	NULL	0	NULL	nephroureterectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients underwent nephroureterectomy and the four got well but one died of acute heart failure .
	manualset3
205296	3	417705	7	NULL	NULL	0	NULL	four	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients underwent nephroureterectomy and the four got well but one died of acute heart failure .
	manualset3
205297	4	417705	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients underwent nephroureterectomy and the four got well but one died of acute heart failure .
	manualset3
205298	5	417705	7	NULL	NULL	0	NULL	acute heart failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients underwent nephroureterectomy and the four got well but one died of acute heart failure .
	manualset3
205299	1	417706	7	NULL	NULL	0	NULL	 supportive birth attendants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Why do supportive birth attendants become directive of maternal bearing-down efforts in second-stage labor ?
	manualset3
205300	2	417706	7	NULL	NULL	0	NULL	maternal bearing-down efforts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Why do supportive birth attendants become directive of maternal bearing-down efforts in second-stage labor ?
	manualset3
205301	3	417706	7	NULL	NULL	0	NULL	second-stage labor	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Why do supportive birth attendants become directive of maternal bearing-down efforts in second-stage labor ?
	manualset3
205302	1	417707	7	NULL	NULL	0	NULL	human cytochrome P450c21	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Why human cytochrome P450c21 is a progesterone 21-hydroxylase .
	manualset3
205303	2	417707	7	NULL	NULL	0	NULL	progesterone 21-hydroxylase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Why human cytochrome P450c21 is a progesterone 21-hydroxylase .
	manualset3
205304	1	417708	7	NULL	NULL	0	NULL	Widal haemagglutination test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Widal and indirect haemagglutination test were used to study the humoral immune response of 45 patients with typhoid fever .
	manualset3
205305	2	417708	7	NULL	NULL	0	NULL	indirect haemagglutination test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Widal and indirect haemagglutination test were used to study the humoral immune response of 45 patients with typhoid fever .
	manualset3
205306	3	417708	7	NULL	NULL	0	NULL	humoral immune response 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Widal and indirect haemagglutination test were used to study the humoral immune response of 45 patients with typhoid fever .
	manualset3
205307	4	417708	7	NULL	NULL	0	NULL	45 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Widal and indirect haemagglutination test were used to study the humoral immune response of 45 patients with typhoid fever .
	manualset3
205308	5	417708	7	NULL	NULL	0	NULL	typhoid fever	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Widal and indirect haemagglutination test were used to study the humoral immune response of 45 patients with typhoid fever .
	manualset3
205309	1	417709	7	NULL	NULL	0	NULL	Wide-ranging frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Wide-ranging frequency preferences of auditory midbrain neurons : Roles of membrane time constant and synaptic properties .
	manualset3
205310	2	417709	7	NULL	NULL	0	NULL	auditory midbrain neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Wide-ranging frequency preferences of auditory midbrain neurons : Roles of membrane time constant and synaptic properties .
	manualset3
205311	3	417709	7	NULL	NULL	0	NULL	Roles	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Wide-ranging frequency preferences of auditory midbrain neurons : Roles of membrane time constant and synaptic properties .
	manualset3
205312	4	417709	7	NULL	NULL	0	NULL	membrane time constant	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Wide-ranging frequency preferences of auditory midbrain neurons : Roles of membrane time constant and synaptic properties .
	manualset3
205313	5	417709	7	NULL	NULL	0	NULL	synaptic properties	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Wide-ranging frequency preferences of auditory midbrain neurons : Roles of membrane time constant and synaptic properties .
	manualset3
205314	1	417710	7	NULL	NULL	0	NULL	Wide-spectrum reconstruction method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Wide-spectrum reconstruction method for a birefringence interference imaging spectrometer .
	manualset3
205315	2	417710	7	NULL	NULL	0	NULL	birefringence interference imaging spectrometer	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Wide-spectrum reconstruction method for a birefringence interference imaging spectrometer .
	manualset3
205316	1	417711	7	NULL	NULL	NULL	NULL	Widely tunable continuous-wave diode-pumped 2-microm Tm-Ho 	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Widely tunable continuous-wave diode-pumped 2-microm Tm-Ho : KYF4 laser .
	manualset3
206954	2	417711	7	NULL	NULL	0	NULL	KYF4 laser	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Widely tunable continuous-wave diode-pumped 2-microm Tm-Ho : KYF4 laser .
	manualset3
205317	1	417712	7	NULL	NULL	0	NULL	mRNA Association	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Widespread mRNA Association with Cytoskeletal Motor Proteins and Identification and Dynamics of Myosin-Associated mRNAs in S. cerevisiae .
	manualset3
205318	2	417712	7	NULL	NULL	0	NULL	Cytoskeletal Motor Proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Widespread mRNA Association with Cytoskeletal Motor Proteins and Identification and Dynamics of Myosin-Associated mRNAs in S. cerevisiae .
	manualset3
205319	3	417712	7	NULL	NULL	0	NULL	Identification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Widespread mRNA Association with Cytoskeletal Motor Proteins and Identification and Dynamics of Myosin-Associated mRNAs in S. cerevisiae .
	manualset3
205320	4	417712	7	NULL	NULL	0	NULL	Dynamics	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Widespread mRNA Association with Cytoskeletal Motor Proteins and Identification and Dynamics of Myosin-Associated mRNAs in S. cerevisiae .
	manualset3
205321	5	417712	7	NULL	NULL	0	NULL	Myosin-Associated mRNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Widespread mRNA Association with Cytoskeletal Motor Proteins and Identification and Dynamics of Myosin-Associated mRNAs in S. cerevisiae .
	manualset3
205322	6	417712	7	NULL	NULL	0	NULL	S. cerevisiae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Widespread mRNA Association with Cytoskeletal Motor Proteins and Identification and Dynamics of Myosin-Associated mRNAs in S. cerevisiae .
	manualset3
205323	1	417713	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients were given the possibility to give a blood test for mercury concentration analysis , but only five were willing to do so .
	manualset3
205324	2	417713	7	NULL	NULL	0	NULL	blood test	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients were given the possibility to give a blood test for mercury concentration analysis , but only five were willing to do so .
	manualset3
205325	3	417713	7	NULL	NULL	0	NULL	mercury concentration analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients were given the possibility to give a blood test for mercury concentration analysis , but only five were willing to do so .
	manualset3
205326	4	417713	7	NULL	NULL	0	NULL	 five	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients were given the possibility to give a blood test for mercury concentration analysis , but only five were willing to do so .
	manualset3
205327	1	417714	7	NULL	NULL	0	NULL	Wild-type RB protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Wild-type RB protein and cyclin A were expressed in both cells .
	manualset3
205328	2	417714	7	NULL	NULL	0	NULL	cyclin A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Wild-type RB protein and cyclin A were expressed in both cells .
	manualset3
205329	3	417714	7	NULL	NULL	0	NULL	 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Wild-type RB protein and cyclin A were expressed in both cells .
	manualset3
205330	1	417715	7	NULL	NULL	0	NULL	Wild-type alpha 1-antitrypsin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Wild-type alpha 1-antitrypsin contains a Met residue at P1 ( position 358 ) , the central position of the reactive center .
	manualset3
205331	2	417715	7	NULL	NULL	0	NULL	Met residue	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Wild-type alpha 1-antitrypsin contains a Met residue at P1 ( position 358 ) , the central position of the reactive center .
	manualset3
205332	3	417715	7	NULL	NULL	0	NULL	P1 ( position 358 )	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Wild-type alpha 1-antitrypsin contains a Met residue at P1 ( position 358 ) , the central position of the reactive center .
	manualset3
205333	4	417715	7	NULL	NULL	NULL	NULL	 central position	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Wild-type alpha 1-antitrypsin contains a Met residue at P1 ( position 358 ) , the central position of the reactive center .
	manualset3
205334	5	417715	7	NULL	NULL	0	NULL	reactive center	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Wild-type alpha 1-antitrypsin contains a Met residue at P1 ( position 358 ) , the central position of the reactive center .
	manualset3
205335	1	417716	7	NULL	NULL	0	NULL	Willebrand factor activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Willebrand factor activity and Willebrand antigen normally increase with age .
	manualset3
205336	2	417716	7	NULL	NULL	NULL	NULL	Willebrand antigen	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Willebrand factor activity and Willebrand antigen normally increase with age .
	manualset3
205337	3	417716	7	NULL	NULL	0	NULL	age	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Willebrand factor activity and Willebrand antigen normally increase with age .
	manualset3
205338	1	417717	7	NULL	NULL	0	NULL	Winter cold 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Winter cold of eastern continental boundaries induced by warm ocean waters .
	manualset3
205339	2	417717	7	NULL	NULL	0	NULL	eastern continental boundaries	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Winter cold of eastern continental boundaries induced by warm ocean waters .
	manualset3
205340	3	417717	7	NULL	NULL	0	NULL	warm ocean waters	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Winter cold of eastern continental boundaries induced by warm ocean waters .
	manualset3
205341	1	417718	7	NULL	NULL	0	NULL	Wireless capsule endoscopy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Wireless capsule endoscopy is one of the recent inventions that has made an impact in the diagnostic work-up of gastrointestinal diseases , mainly in small intestinal pathology , the part of the gut that can not be totally visualized by upper and lower gastrointestinal endoscopy .
	manualset3
205342	2	417718	7	NULL	NULL	0	NULL	inventions	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Wireless capsule endoscopy is one of the recent inventions that has made an impact in the diagnostic work-up of gastrointestinal diseases , mainly in small intestinal pathology , the part of the gut that can not be totally visualized by upper and lower gastrointestinal endoscopy .
	manualset3
205343	3	417718	7	NULL	NULL	0	NULL	 impact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Wireless capsule endoscopy is one of the recent inventions that has made an impact in the diagnostic work-up of gastrointestinal diseases , mainly in small intestinal pathology , the part of the gut that can not be totally visualized by upper and lower gastrointestinal endoscopy .
	manualset3
205344	4	417718	7	NULL	NULL	0	NULL	diagnostic work-up	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Wireless capsule endoscopy is one of the recent inventions that has made an impact in the diagnostic work-up of gastrointestinal diseases , mainly in small intestinal pathology , the part of the gut that can not be totally visualized by upper and lower gastrointestinal endoscopy .
	manualset3
205345	5	417718	7	NULL	NULL	0	NULL	gastrointestinal diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Wireless capsule endoscopy is one of the recent inventions that has made an impact in the diagnostic work-up of gastrointestinal diseases , mainly in small intestinal pathology , the part of the gut that can not be totally visualized by upper and lower gastrointestinal endoscopy .
	manualset3
205346	6	417718	7	NULL	NULL	0	NULL	small intestinal pathology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Wireless capsule endoscopy is one of the recent inventions that has made an impact in the diagnostic work-up of gastrointestinal diseases , mainly in small intestinal pathology , the part of the gut that can not be totally visualized by upper and lower gastrointestinal endoscopy .
	manualset3
205347	7	417718	7	NULL	NULL	0	NULL	part of the gut	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Wireless capsule endoscopy is one of the recent inventions that has made an impact in the diagnostic work-up of gastrointestinal diseases , mainly in small intestinal pathology , the part of the gut that can not be totally visualized by upper and lower gastrointestinal endoscopy .
	manualset3
205348	8	417718	7	NULL	NULL	0	NULL	upper gastrointestinal endoscopy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Wireless capsule endoscopy is one of the recent inventions that has made an impact in the diagnostic work-up of gastrointestinal diseases , mainly in small intestinal pathology , the part of the gut that can not be totally visualized by upper and lower gastrointestinal endoscopy .
	manualset3
205349	9	417718	7	NULL	NULL	0	NULL	lower gastrointestinal endoscopy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Wireless capsule endoscopy is one of the recent inventions that has made an impact in the diagnostic work-up of gastrointestinal diseases , mainly in small intestinal pathology , the part of the gut that can not be totally visualized by upper and lower gastrointestinal endoscopy .
	manualset3
205350	1	417719	7	NULL	NULL	0	NULL	Wistar rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Wistar rats acclimated to cold received iv 25 micrograms T 4/100 g bw , 21 micrograms T 3/100 g bw or 2.5 micrograms T 3/100 g bw , to observe the changes induced in the peripheral metabolism of 125I-T4 and 125I-T3 relative to cold-adapted untreated animals .
	manualset3
205351	2	417719	7	NULL	NULL	0	NULL	cold	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Wistar rats acclimated to cold received iv 25 micrograms T 4/100 g bw , 21 micrograms T 3/100 g bw or 2.5 micrograms T 3/100 g bw , to observe the changes induced in the peripheral metabolism of 125I-T4 and 125I-T3 relative to cold-adapted untreated animals .
	manualset3
205352	3	417719	7	NULL	NULL	0	NULL	iv 25 micrograms	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Wistar rats acclimated to cold received iv 25 micrograms T 4/100 g bw , 21 micrograms T 3/100 g bw or 2.5 micrograms T 3/100 g bw , to observe the changes induced in the peripheral metabolism of 125I-T4 and 125I-T3 relative to cold-adapted untreated animals .
	manualset3
205353	4	417719	7	NULL	NULL	0	NULL	T 4/100 g bw	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Wistar rats acclimated to cold received iv 25 micrograms T 4/100 g bw , 21 micrograms T 3/100 g bw or 2.5 micrograms T 3/100 g bw , to observe the changes induced in the peripheral metabolism of 125I-T4 and 125I-T3 relative to cold-adapted untreated animals .
	manualset3
205354	5	417719	7	NULL	NULL	0	NULL	21 micrograms	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Wistar rats acclimated to cold received iv 25 micrograms T 4/100 g bw , 21 micrograms T 3/100 g bw or 2.5 micrograms T 3/100 g bw , to observe the changes induced in the peripheral metabolism of 125I-T4 and 125I-T3 relative to cold-adapted untreated animals .
	manualset3
205355	6	417719	7	NULL	NULL	0	NULL	T 3/100 g bw	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Wistar rats acclimated to cold received iv 25 micrograms T 4/100 g bw , 21 micrograms T 3/100 g bw or 2.5 micrograms T 3/100 g bw , to observe the changes induced in the peripheral metabolism of 125I-T4 and 125I-T3 relative to cold-adapted untreated animals .
	manualset3
205356	7	417719	7	NULL	NULL	0	NULL	2.5 micrograms	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Wistar rats acclimated to cold received iv 25 micrograms T 4/100 g bw , 21 micrograms T 3/100 g bw or 2.5 micrograms T 3/100 g bw , to observe the changes induced in the peripheral metabolism of 125I-T4 and 125I-T3 relative to cold-adapted untreated animals .
	manualset3
205357	8	417719	7	NULL	NULL	0	NULL	T 3/100 g bw	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Wistar rats acclimated to cold received iv 25 micrograms T 4/100 g bw , 21 micrograms T 3/100 g bw or 2.5 micrograms T 3/100 g bw , to observe the changes induced in the peripheral metabolism of 125I-T4 and 125I-T3 relative to cold-adapted untreated animals .
	manualset3
205358	9	417719	7	NULL	NULL	0	NULL	changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Wistar rats acclimated to cold received iv 25 micrograms T 4/100 g bw , 21 micrograms T 3/100 g bw or 2.5 micrograms T 3/100 g bw , to observe the changes induced in the peripheral metabolism of 125I-T4 and 125I-T3 relative to cold-adapted untreated animals .
	manualset3
205359	10	417719	7	NULL	NULL	0	NULL	peripheral metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Wistar rats acclimated to cold received iv 25 micrograms T 4/100 g bw , 21 micrograms T 3/100 g bw or 2.5 micrograms T 3/100 g bw , to observe the changes induced in the peripheral metabolism of 125I-T4 and 125I-T3 relative to cold-adapted untreated animals .
	manualset3
205360	11	417719	7	NULL	NULL	NULL	NULL	125I-T4	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Wistar rats acclimated to cold received iv 25 micrograms T 4/100 g bw , 21 micrograms T 3/100 g bw or 2.5 micrograms T 3/100 g bw , to observe the changes induced in the peripheral metabolism of 125I-T4 and 125I-T3 relative to cold-adapted untreated animals .
	manualset3
205361	12	417719	7	NULL	NULL	0	NULL	125I-T3	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Wistar rats acclimated to cold received iv 25 micrograms T 4/100 g bw , 21 micrograms T 3/100 g bw or 2.5 micrograms T 3/100 g bw , to observe the changes induced in the peripheral metabolism of 125I-T4 and 125I-T3 relative to cold-adapted untreated animals .
	manualset3
205362	13	417719	7	NULL	NULL	0	NULL	cold-adapted untreated animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Wistar rats acclimated to cold received iv 25 micrograms T 4/100 g bw , 21 micrograms T 3/100 g bw or 2.5 micrograms T 3/100 g bw , to observe the changes induced in the peripheral metabolism of 125I-T4 and 125I-T3 relative to cold-adapted untreated animals .
	manualset3
205363	1	417720	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients were relieved of symptoms and returned to work , one of whom relapsed two years later to undergo reoperation .
	manualset3
205364	2	417720	7	NULL	NULL	0	NULL	symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients were relieved of symptoms and returned to work , one of whom relapsed two years later to undergo reoperation .
	manualset3
205365	3	417720	7	NULL	NULL	0	NULL	work	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients were relieved of symptoms and returned to work , one of whom relapsed two years later to undergo reoperation .
	manualset3
205366	4	417720	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients were relieved of symptoms and returned to work , one of whom relapsed two years later to undergo reoperation .
	manualset3
205367	5	417720	7	NULL	NULL	0	NULL	two years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients were relieved of symptoms and returned to work , one of whom relapsed two years later to undergo reoperation .
	manualset3
205368	6	417720	7	NULL	NULL	0	NULL	reoperation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients were relieved of symptoms and returned to work , one of whom relapsed two years later to undergo reoperation .
	manualset3
205369	1	417721	7	NULL	NULL	0	NULL	AtOPT4	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	With AtOPT4 , initially only small KLGL-dependent currents were recorded in batches of oocytes showing high ScOPT1 expression .
	manualset3
205370	2	417721	7	NULL	NULL	0	NULL	small KLGL-dependent currents	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	With AtOPT4 , initially only small KLGL-dependent currents were recorded in batches of oocytes showing high ScOPT1 expression .
	manualset3
205372	3	417721	7	NULL	NULL	0	NULL	 batches	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	With AtOPT4 , initially only small KLGL-dependent currents were recorded in batches of oocytes showing high ScOPT1 expression .
	manualset3
205374	4	417721	7	NULL	NULL	0	NULL	oocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	With AtOPT4 , initially only small KLGL-dependent currents were recorded in batches of oocytes showing high ScOPT1 expression .
	manualset3
205376	5	417721	7	NULL	NULL	0	NULL	high ScOPT1 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	With AtOPT4 , initially only small KLGL-dependent currents were recorded in batches of oocytes showing high ScOPT1 expression .
	manualset3
205381	1	417722	7	NULL	NULL	0	NULL	PTH + GN	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	With PTH + GN no further decrease was observed .
	manualset3
205382	1	417723	7	NULL	NULL	0	NULL	system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	With a system based on an original computer program for the compiling , store and process essential data on cancer diseases we analyzed 736 consecutive and unselected oral carcinomas and we studied the prognostic value of main clinical factors .
	manualset3
205383	2	417723	7	NULL	NULL	0	NULL	original computer program	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	With a system based on an original computer program for the compiling , store and process essential data on cancer diseases we analyzed 736 consecutive and unselected oral carcinomas and we studied the prognostic value of main clinical factors .
	manualset3
205384	3	417723	7	NULL	NULL	0	NULL	essential data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	With a system based on an original computer program for the compiling , store and process essential data on cancer diseases we analyzed 736 consecutive and unselected oral carcinomas and we studied the prognostic value of main clinical factors .
	manualset3
205385	4	417723	7	NULL	NULL	0	NULL	cancer diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	With a system based on an original computer program for the compiling , store and process essential data on cancer diseases we analyzed 736 consecutive and unselected oral carcinomas and we studied the prognostic value of main clinical factors .
	manualset3
205386	5	417723	7	NULL	NULL	0	NULL	736 consecutive oral carcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	With a system based on an original computer program for the compiling , store and process essential data on cancer diseases we analyzed 736 consecutive and unselected oral carcinomas and we studied the prognostic value of main clinical factors .
	manualset3
205387	6	417723	7	NULL	NULL	0	NULL	unselected oral carcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	With a system based on an original computer program for the compiling , store and process essential data on cancer diseases we analyzed 736 consecutive and unselected oral carcinomas and we studied the prognostic value of main clinical factors .
	manualset3
205388	7	417723	7	NULL	NULL	0	NULL	prognostic value	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With a system based on an original computer program for the compiling , store and process essential data on cancer diseases we analyzed 736 consecutive and unselected oral carcinomas and we studied the prognostic value of main clinical factors .
	manualset3
205389	8	417723	7	NULL	NULL	0	NULL	main clinical factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	With a system based on an original computer program for the compiling , store and process essential data on cancer diseases we analyzed 736 consecutive and unselected oral carcinomas and we studied the prognostic value of main clinical factors .
	manualset3
205394	1	417724	7	NULL	NULL	0	NULL	three-dimensional optical-tweezers trap	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	With a three-dimensional optical-tweezers trap , a single sperm was caught and transported through the laser-drilled hole directly into the perivitelline space .
	manualset3
205395	2	417724	7	NULL	NULL	0	NULL	single sperm	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	With a three-dimensional optical-tweezers trap , a single sperm was caught and transported through the laser-drilled hole directly into the perivitelline space .
	manualset3
205398	3	417724	7	NULL	NULL	0	NULL	laser-drilled hole	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	With a three-dimensional optical-tweezers trap , a single sperm was caught and transported through the laser-drilled hole directly into the perivitelline space .
	manualset3
205399	4	417724	7	NULL	NULL	0	NULL	perivitelline space 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	With a three-dimensional optical-tweezers trap , a single sperm was caught and transported through the laser-drilled hole directly into the perivitelline space .
	manualset3
205402	1	417725	7	NULL	NULL	0	NULL	Le ( y ) based vaccines	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	With a view to developing Le ( y ) based vaccines we have examined the immunogenicity of Le ( y ) - protein conjugates in mice .
	manualset3
205403	2	417725	7	NULL	NULL	0	NULL	immunogenicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With a view to developing Le ( y ) based vaccines we have examined the immunogenicity of Le ( y ) - protein conjugates in mice .
	manualset3
205404	3	417725	7	NULL	NULL	0	NULL	Le ( y ) - protein conjugates	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	With a view to developing Le ( y ) based vaccines we have examined the immunogenicity of Le ( y ) - protein conjugates in mice .
	manualset3
205405	4	417725	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	With a view to developing Le ( y ) based vaccines we have examined the immunogenicity of Le ( y ) - protein conjugates in mice .
	manualset3
205409	1	417726	7	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	With adequate therapy he recovered after a few days .
	manualset3
205410	2	417726	7	NULL	NULL	0	NULL	 few days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	With adequate therapy he recovered after a few days .
	manualset3
205411	1	417727	7	NULL	NULL	0	NULL	aging	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	With aging , the brain undergoes neuronal loss in many areas .
	manualset3
205412	2	417727	7	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	With aging , the brain undergoes neuronal loss in many areas .
	manualset3
205413	3	417727	7	NULL	NULL	0	NULL	neuronal loss	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	With aging , the brain undergoes neuronal loss in many areas .
	manualset3
205414	4	417727	7	NULL	NULL	0	NULL	 areas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	With aging , the brain undergoes neuronal loss in many areas .
	manualset3
205415	1	417728	7	NULL	NULL	0	NULL	 increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With an increase in the degree of oxidation , Ox-LDL was more retained on the DEAE-glucomannan gel with a concomitant increase in the CL intensity .
	manualset3
205416	2	417728	7	NULL	NULL	0	NULL	degree	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With an increase in the degree of oxidation , Ox-LDL was more retained on the DEAE-glucomannan gel with a concomitant increase in the CL intensity .
	manualset3
205417	3	417728	7	NULL	NULL	0	NULL	oxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	With an increase in the degree of oxidation , Ox-LDL was more retained on the DEAE-glucomannan gel with a concomitant increase in the CL intensity .
	manualset3
205418	4	417728	7	NULL	NULL	0	NULL	Ox-LDL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	With an increase in the degree of oxidation , Ox-LDL was more retained on the DEAE-glucomannan gel with a concomitant increase in the CL intensity .
	manualset3
205419	5	417728	7	NULL	NULL	0	NULL	DEAE-glucomannan gel 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	With an increase in the degree of oxidation , Ox-LDL was more retained on the DEAE-glucomannan gel with a concomitant increase in the CL intensity .
	manualset3
205420	6	417728	7	NULL	NULL	0	NULL	 increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With an increase in the degree of oxidation , Ox-LDL was more retained on the DEAE-glucomannan gel with a concomitant increase in the CL intensity .
	manualset3
205421	7	417728	7	NULL	NULL	0	NULL	CL intensity	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	With an increase in the degree of oxidation , Ox-LDL was more retained on the DEAE-glucomannan gel with a concomitant increase in the CL intensity .
	manualset3
205425	1	417729	7	NULL	NULL	0	NULL	aortic clamping	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	With aortic clamping alone , ICP increased from 9.8 + / - 2.2 mm Hg to 15.2 + / - 2.8 mm Hg ( p & lt ; 0.05 ) .
	manualset3
205426	2	417729	7	NULL	NULL	0	NULL	ICP	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With aortic clamping alone , ICP increased from 9.8 + / - 2.2 mm Hg to 15.2 + / - 2.8 mm Hg ( p & lt ; 0.05 ) .
	manualset3
205427	3	417729	7	NULL	NULL	0	NULL	9.8 + / - 2.2 mm Hg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	With aortic clamping alone , ICP increased from 9.8 + / - 2.2 mm Hg to 15.2 + / - 2.8 mm Hg ( p & lt ; 0.05 ) .
	manualset3
205429	4	417729	7	NULL	NULL	0	NULL	15.2 + / - 2.8 mm Hg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	With aortic clamping alone , ICP increased from 9.8 + / - 2.2 mm Hg to 15.2 + / - 2.8 mm Hg ( p & lt ; 0.05 ) .
	manualset3
205434	5	417729	7	NULL	NULL	0	NULL	p & lt ; 0.05	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With aortic clamping alone , ICP increased from 9.8 + / - 2.2 mm Hg to 15.2 + / - 2.8 mm Hg ( p & lt ; 0.05 ) .
	manualset3
205437	1	417730	7	NULL	NULL	0	NULL	scales	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With both scales there was a large intersubject variation in the relationship between dyspnoea score and minute ventilation ( VE ) ( P less than 0.01 ) , and in the range of the scale used .
	manualset3
205438	2	417730	7	NULL	NULL	0	NULL	large intersubject variation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With both scales there was a large intersubject variation in the relationship between dyspnoea score and minute ventilation ( VE ) ( P less than 0.01 ) , and in the range of the scale used .
	manualset3
205439	3	417730	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	With both scales there was a large intersubject variation in the relationship between dyspnoea score and minute ventilation ( VE ) ( P less than 0.01 ) , and in the range of the scale used .
	manualset3
205440	4	417730	7	NULL	NULL	0	NULL	dyspnoea score	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With both scales there was a large intersubject variation in the relationship between dyspnoea score and minute ventilation ( VE ) ( P less than 0.01 ) , and in the range of the scale used .
	manualset3
205441	5	417730	7	NULL	NULL	0	NULL	minute ventilation ( VE )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	With both scales there was a large intersubject variation in the relationship between dyspnoea score and minute ventilation ( VE ) ( P less than 0.01 ) , and in the range of the scale used .
	manualset3
205442	6	417730	7	NULL	NULL	0	NULL	P less than 0.01	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With both scales there was a large intersubject variation in the relationship between dyspnoea score and minute ventilation ( VE ) ( P less than 0.01 ) , and in the range of the scale used .
	manualset3
205443	7	417730	7	NULL	NULL	0	NULL	 range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With both scales there was a large intersubject variation in the relationship between dyspnoea score and minute ventilation ( VE ) ( P less than 0.01 ) , and in the range of the scale used .
	manualset3
205444	8	417730	7	NULL	NULL	0	NULL	scale	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With both scales there was a large intersubject variation in the relationship between dyspnoea score and minute ventilation ( VE ) ( P less than 0.01 ) , and in the range of the scale used .
	manualset3
205445	1	417731	7	NULL	NULL	0	NULL	dissociation constants ( KD )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With dissociation constants ( KD ) of ( 3H ) AMPA binding and inhibition concentrations ( IC50 ) of L-BOAA , 6-OH-DOPA and L-glutamate obtained from saturation and displacement experiments inhibition constants ( Ki ) for the inhibition of ( 3H ) AMPA binding in individual hippocampal subregions could be calculated .
	manualset3
205446	2	417731	7	NULL	NULL	0	NULL	( 3H ) AMPA binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	With dissociation constants ( KD ) of ( 3H ) AMPA binding and inhibition concentrations ( IC50 ) of L-BOAA , 6-OH-DOPA and L-glutamate obtained from saturation and displacement experiments inhibition constants ( Ki ) for the inhibition of ( 3H ) AMPA binding in individual hippocampal subregions could be calculated .
	manualset3
205447	3	417731	7	NULL	NULL	NULL	NULL	inhibition concentrations ( IC50 )	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	With dissociation constants ( KD ) of ( 3H ) AMPA binding and inhibition concentrations ( IC50 ) of L-BOAA , 6-OH-DOPA and L-glutamate obtained from saturation and displacement experiments inhibition constants ( Ki ) for the inhibition of ( 3H ) AMPA binding in individual hippocampal subregions could be calculated .
	manualset3
205448	4	417731	7	NULL	NULL	0	NULL	L-BOAA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	With dissociation constants ( KD ) of ( 3H ) AMPA binding and inhibition concentrations ( IC50 ) of L-BOAA , 6-OH-DOPA and L-glutamate obtained from saturation and displacement experiments inhibition constants ( Ki ) for the inhibition of ( 3H ) AMPA binding in individual hippocampal subregions could be calculated .
	manualset3
205449	5	417731	7	NULL	NULL	0	NULL	6-OH-DOPA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	With dissociation constants ( KD ) of ( 3H ) AMPA binding and inhibition concentrations ( IC50 ) of L-BOAA , 6-OH-DOPA and L-glutamate obtained from saturation and displacement experiments inhibition constants ( Ki ) for the inhibition of ( 3H ) AMPA binding in individual hippocampal subregions could be calculated .
	manualset3
205450	6	417731	7	NULL	NULL	0	NULL	L-glutamate	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	With dissociation constants ( KD ) of ( 3H ) AMPA binding and inhibition concentrations ( IC50 ) of L-BOAA , 6-OH-DOPA and L-glutamate obtained from saturation and displacement experiments inhibition constants ( Ki ) for the inhibition of ( 3H ) AMPA binding in individual hippocampal subregions could be calculated .
	manualset3
205451	7	417731	7	NULL	NULL	0	NULL	saturation and displacement experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	With dissociation constants ( KD ) of ( 3H ) AMPA binding and inhibition concentrations ( IC50 ) of L-BOAA , 6-OH-DOPA and L-glutamate obtained from saturation and displacement experiments inhibition constants ( Ki ) for the inhibition of ( 3H ) AMPA binding in individual hippocampal subregions could be calculated .
	manualset3
205452	8	417731	7	NULL	NULL	0	NULL	inhibition constants ( Ki )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With dissociation constants ( KD ) of ( 3H ) AMPA binding and inhibition concentrations ( IC50 ) of L-BOAA , 6-OH-DOPA and L-glutamate obtained from saturation and displacement experiments inhibition constants ( Ki ) for the inhibition of ( 3H ) AMPA binding in individual hippocampal subregions could be calculated .
	manualset3
205453	9	417731	7	NULL	NULL	0	NULL	 inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	With dissociation constants ( KD ) of ( 3H ) AMPA binding and inhibition concentrations ( IC50 ) of L-BOAA , 6-OH-DOPA and L-glutamate obtained from saturation and displacement experiments inhibition constants ( Ki ) for the inhibition of ( 3H ) AMPA binding in individual hippocampal subregions could be calculated .
	manualset3
205454	10	417731	7	NULL	NULL	0	NULL	( 3H ) AMPA binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	With dissociation constants ( KD ) of ( 3H ) AMPA binding and inhibition concentrations ( IC50 ) of L-BOAA , 6-OH-DOPA and L-glutamate obtained from saturation and displacement experiments inhibition constants ( Ki ) for the inhibition of ( 3H ) AMPA binding in individual hippocampal subregions could be calculated .
	manualset3
205455	11	417731	7	NULL	NULL	0	NULL	hippocampal subregions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	With dissociation constants ( KD ) of ( 3H ) AMPA binding and inhibition concentrations ( IC50 ) of L-BOAA , 6-OH-DOPA and L-glutamate obtained from saturation and displacement experiments inhibition constants ( Ki ) for the inhibition of ( 3H ) AMPA binding in individual hippocampal subregions could be calculated .
	manualset3
205456	1	417732	7	NULL	NULL	0	NULL	dual beam flow cytometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	With dual beam flow cytometry , both the amount of hybridized probe and the DNA content of individual nuclei were determined .
	manualset3
205457	2	417732	7	NULL	NULL	0	NULL	 amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With dual beam flow cytometry , both the amount of hybridized probe and the DNA content of individual nuclei were determined .
	manualset3
205458	3	417732	7	NULL	NULL	0	NULL	hybridized probe	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	With dual beam flow cytometry , both the amount of hybridized probe and the DNA content of individual nuclei were determined .
	manualset3
205459	4	417732	7	NULL	NULL	0	NULL	DNA content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With dual beam flow cytometry , both the amount of hybridized probe and the DNA content of individual nuclei were determined .
	manualset3
205460	5	417732	7	NULL	NULL	0	NULL	individual nuclei	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	With dual beam flow cytometry , both the amount of hybridized probe and the DNA content of individual nuclei were determined .
	manualset3
205524	1	417733	7	NULL	NULL	0	NULL	dynamic recovery	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With dynamic recovery ( 6.0 days ) , they increased acceptance to ) 80 % of preconditioning levels .
	manualset3
205525	2	417733	7	NULL	NULL	0	NULL	6.0 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	With dynamic recovery ( 6.0 days ) , they increased acceptance to ) 80 % of preconditioning levels .
	manualset3
205526	3	417733	7	NULL	NULL	0	NULL	acceptance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With dynamic recovery ( 6.0 days ) , they increased acceptance to ) 80 % of preconditioning levels .
	manualset3
205527	4	417733	7	NULL	NULL	0	NULL	80 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With dynamic recovery ( 6.0 days ) , they increased acceptance to ) 80 % of preconditioning levels .
	manualset3
205528	5	417733	7	NULL	NULL	0	NULL	 preconditioning levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With dynamic recovery ( 6.0 days ) , they increased acceptance to ) 80 % of preconditioning levels .
	manualset3
205566	1	417734	7	NULL	NULL	0	NULL	sensor	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	With either sensor , basal cellular fluorescence emission centered near 470 nm , indicative of sensor-Zn-proteins .
	manualset3
205567	2	417734	7	NULL	NULL	0	NULL	basal cellular fluorescence emission 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With either sensor , basal cellular fluorescence emission centered near 470 nm , indicative of sensor-Zn-proteins .
	manualset3
205568	3	417734	7	NULL	NULL	0	NULL	470 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	With either sensor , basal cellular fluorescence emission centered near 470 nm , indicative of sensor-Zn-proteins .
	manualset3
205570	4	417734	7	NULL	NULL	0	NULL	sensor-Zn-proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	With either sensor , basal cellular fluorescence emission centered near 470 nm , indicative of sensor-Zn-proteins .
	manualset3
205572	1	417735	7	NULL	NULL	0	NULL	polymers	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All polymers showed higher rates of drug release at higher pH values ( 9.0 ) 7.4 ) 2.0 ) and at higher temperatures ( 37 degrees C ) 20 degrees C ) .
	manualset3
205573	2	417735	7	NULL	NULL	0	NULL	higher rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All polymers showed higher rates of drug release at higher pH values ( 9.0 ) 7.4 ) 2.0 ) and at higher temperatures ( 37 degrees C ) 20 degrees C ) .
	manualset3
205575	3	417735	7	NULL	NULL	0	NULL	drug release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All polymers showed higher rates of drug release at higher pH values ( 9.0 ) 7.4 ) 2.0 ) and at higher temperatures ( 37 degrees C ) 20 degrees C ) .
	manualset3
205576	4	417735	7	NULL	NULL	0	NULL	pH values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All polymers showed higher rates of drug release at higher pH values ( 9.0 ) 7.4 ) 2.0 ) and at higher temperatures ( 37 degrees C ) 20 degrees C ) .
	manualset3
205577	5	417735	7	NULL	NULL	0	NULL	( 9.0 ) 7.4 ) 2.0 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	All polymers showed higher rates of drug release at higher pH values ( 9.0 ) 7.4 ) 2.0 ) and at higher temperatures ( 37 degrees C ) 20 degrees C ) .
	manualset3
205578	6	417735	7	NULL	NULL	0	NULL	higher temperatures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All polymers showed higher rates of drug release at higher pH values ( 9.0 ) 7.4 ) 2.0 ) and at higher temperatures ( 37 degrees C ) 20 degrees C ) .
	manualset3
205579	7	417735	7	NULL	NULL	0	NULL	 37 degrees C	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All polymers showed higher rates of drug release at higher pH values ( 9.0 ) 7.4 ) 2.0 ) and at higher temperatures ( 37 degrees C ) 20 degrees C ) .
	manualset3
205580	8	417735	7	NULL	NULL	0	NULL	20 degrees C	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All polymers showed higher rates of drug release at higher pH values ( 9.0 ) 7.4 ) 2.0 ) and at higher temperatures ( 37 degrees C ) 20 degrees C ) .
	manualset3
205610	1	417736	7	NULL	NULL	0	NULL	emerging technology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	With emerging technology driving all medical disciplines and the rapid pace at which it emerges , it is vital for the contemporary practitioner to keep abreast of the newest information technology developments .
	manualset3
205611	2	417736	7	NULL	NULL	0	NULL	medical disciplines	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	With emerging technology driving all medical disciplines and the rapid pace at which it emerges , it is vital for the contemporary practitioner to keep abreast of the newest information technology developments .
	manualset3
205612	3	417736	7	NULL	NULL	0	NULL	 rapid pace	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With emerging technology driving all medical disciplines and the rapid pace at which it emerges , it is vital for the contemporary practitioner to keep abreast of the newest information technology developments .
	manualset3
205614	4	417736	7	NULL	NULL	0	NULL	vital	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With emerging technology driving all medical disciplines and the rapid pace at which it emerges , it is vital for the contemporary practitioner to keep abreast of the newest information technology developments .
	manualset3
205615	5	417736	7	NULL	NULL	0	NULL	contemporary practitioner	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	With emerging technology driving all medical disciplines and the rapid pace at which it emerges , it is vital for the contemporary practitioner to keep abreast of the newest information technology developments .
	manualset3
205617	6	417736	7	NULL	NULL	0	NULL	newest information technology developments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With emerging technology driving all medical disciplines and the rapid pace at which it emerges , it is vital for the contemporary practitioner to keep abreast of the newest information technology developments .
	manualset3
205620	1	417737	7	NULL	NULL	0	NULL	excitation wavelength	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With excitation wavelength at 254 nm , the maximum emission wavelengths of carvedilol and ampicillin sodium were at 357 and 426 nm , respectively .
	manualset3
205621	2	417737	7	NULL	NULL	0	NULL	254 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	With excitation wavelength at 254 nm , the maximum emission wavelengths of carvedilol and ampicillin sodium were at 357 and 426 nm , respectively .
	manualset3
205624	3	417737	7	NULL	NULL	0	NULL	 maximum emission wavelengths	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With excitation wavelength at 254 nm , the maximum emission wavelengths of carvedilol and ampicillin sodium were at 357 and 426 nm , respectively .
	manualset3
205626	4	417737	7	NULL	NULL	NULL	NULL	carvedilol 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	With excitation wavelength at 254 nm , the maximum emission wavelengths of carvedilol and ampicillin sodium were at 357 and 426 nm , respectively .
	manualset3
205628	5	417737	7	NULL	NULL	0	NULL	ampicillin sodium	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	With excitation wavelength at 254 nm , the maximum emission wavelengths of carvedilol and ampicillin sodium were at 357 and 426 nm , respectively .
	manualset3
205629	6	417737	7	NULL	NULL	0	NULL	357 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	With excitation wavelength at 254 nm , the maximum emission wavelengths of carvedilol and ampicillin sodium were at 357 and 426 nm , respectively .
	manualset3
205630	7	417737	7	NULL	NULL	0	NULL	426 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	With excitation wavelength at 254 nm , the maximum emission wavelengths of carvedilol and ampicillin sodium were at 357 and 426 nm , respectively .
	manualset3
205634	1	417738	7	NULL	NULL	0	NULL	exceptions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With few exceptions , established breast cancer risk factors were similarly associated with risk of death from breast cancer among African-American women and White women .
	manualset3
205649	2	417738	7	NULL	NULL	NULL	NULL	breast cancer risk factors	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	With few exceptions , established breast cancer risk factors were similarly associated with risk of death from breast cancer among African-American women and White women .
	manualset3
205650	3	417738	7	NULL	NULL	NULL	NULL	 risk of death	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	With few exceptions , established breast cancer risk factors were similarly associated with risk of death from breast cancer among African-American women and White women .
	manualset3
205651	4	417738	7	NULL	NULL	0	NULL	breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	With few exceptions , established breast cancer risk factors were similarly associated with risk of death from breast cancer among African-American women and White women .
	manualset3
205652	5	417738	7	NULL	NULL	0	NULL	African-American women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	With few exceptions , established breast cancer risk factors were similarly associated with risk of death from breast cancer among African-American women and White women .
	manualset3
205653	6	417738	7	NULL	NULL	0	NULL	White women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	With few exceptions , established breast cancer risk factors were similarly associated with risk of death from breast cancer among African-American women and White women .
	manualset3
205654	1	417739	7	NULL	NULL	0	NULL	first-row transition metal ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	With first-row transition metal ions , L tends to form binuclear complexes but , depending on the nature of the particular metal ion , the structure of the binuclear complex may be very different .
	manualset3
205655	2	417739	7	NULL	NULL	0	NULL	 L 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	With first-row transition metal ions , L tends to form binuclear complexes but , depending on the nature of the particular metal ion , the structure of the binuclear complex may be very different .
	manualset3
205656	3	417739	7	NULL	NULL	0	NULL	binuclear complexes	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	With first-row transition metal ions , L tends to form binuclear complexes but , depending on the nature of the particular metal ion , the structure of the binuclear complex may be very different .
	manualset3
205657	4	417739	7	NULL	NULL	0	NULL	metal ion	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	With first-row transition metal ions , L tends to form binuclear complexes but , depending on the nature of the particular metal ion , the structure of the binuclear complex may be very different .
	manualset3
205658	5	417739	7	NULL	NULL	0	NULL	structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	With first-row transition metal ions , L tends to form binuclear complexes but , depending on the nature of the particular metal ion , the structure of the binuclear complex may be very different .
	manualset3
205659	6	417739	7	NULL	NULL	0	NULL	binuclear complex	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	With first-row transition metal ions , L tends to form binuclear complexes but , depending on the nature of the particular metal ion , the structure of the binuclear complex may be very different .
	manualset3
205660	7	417739	7	NULL	NULL	0	NULL	nature	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With first-row transition metal ions , L tends to form binuclear complexes but , depending on the nature of the particular metal ion , the structure of the binuclear complex may be very different .
	manualset3
205661	1	417740	7	NULL	NULL	0	NULL	increasing nitrogen fertilization rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With increasing nitrogen fertilization rate , the protein and lysine contents of the grains increased , while the starch content decreased .
	manualset3
205662	2	417740	7	NULL	NULL	0	NULL	 protein contents	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With increasing nitrogen fertilization rate , the protein and lysine contents of the grains increased , while the starch content decreased .
	manualset3
205663	3	417740	7	NULL	NULL	0	NULL	lysine contents	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With increasing nitrogen fertilization rate , the protein and lysine contents of the grains increased , while the starch content decreased .
	manualset3
205664	4	417740	7	NULL	NULL	0	NULL	grains	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	With increasing nitrogen fertilization rate , the protein and lysine contents of the grains increased , while the starch content decreased .
	manualset3
205665	5	417740	7	NULL	NULL	0	NULL	starch content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With increasing nitrogen fertilization rate , the protein and lysine contents of the grains increased , while the starch content decreased .
	manualset3
205666	1	417741	7	NULL	NULL	0	NULL	information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	With information now available it is possible to identify some of the reasons why these trials have failed to answer the fundamentally important question of whether the drugs can modify the long-term course of RA .
	manualset3
205667	2	417741	7	NULL	NULL	0	NULL	reasons 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With information now available it is possible to identify some of the reasons why these trials have failed to answer the fundamentally important question of whether the drugs can modify the long-term course of RA .
	manualset3
205694	3	417741	7	NULL	NULL	0	NULL	trials	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	With information now available it is possible to identify some of the reasons why these trials have failed to answer the fundamentally important question of whether the drugs can modify the long-term course of RA .
	manualset3
205695	4	417741	7	NULL	NULL	0	NULL	question	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	With information now available it is possible to identify some of the reasons why these trials have failed to answer the fundamentally important question of whether the drugs can modify the long-term course of RA .
	manualset3
205696	5	417741	7	NULL	NULL	0	NULL	drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	With information now available it is possible to identify some of the reasons why these trials have failed to answer the fundamentally important question of whether the drugs can modify the long-term course of RA .
	manualset3
205697	6	417741	7	NULL	NULL	0	NULL	long-term course 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	With information now available it is possible to identify some of the reasons why these trials have failed to answer the fundamentally important question of whether the drugs can modify the long-term course of RA .
	manualset3
205698	7	417741	7	NULL	NULL	0	NULL	RA	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	With information now available it is possible to identify some of the reasons why these trials have failed to answer the fundamentally important question of whether the drugs can modify the long-term course of RA .
	manualset3
205699	1	417742	7	NULL	NULL	0	NULL	lecithin phosphorus concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With lecithin phosphorus concentration as the reference standard , the predictive value of a mature Amniostat-FLM result was 96.2 % , whereas that of an immature result was 58.5 % .
	manualset3
205700	2	417742	7	NULL	NULL	0	NULL	reference standard	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	With lecithin phosphorus concentration as the reference standard , the predictive value of a mature Amniostat-FLM result was 96.2 % , whereas that of an immature result was 58.5 % .
	manualset3
205701	3	417742	7	NULL	NULL	0	NULL	predictive value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With lecithin phosphorus concentration as the reference standard , the predictive value of a mature Amniostat-FLM result was 96.2 % , whereas that of an immature result was 58.5 % .
	manualset3
205702	4	417742	7	NULL	NULL	0	NULL	mature Amniostat-FLM result	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With lecithin phosphorus concentration as the reference standard , the predictive value of a mature Amniostat-FLM result was 96.2 % , whereas that of an immature result was 58.5 % .
	manualset3
205703	5	417742	7	NULL	NULL	0	NULL	96.2 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With lecithin phosphorus concentration as the reference standard , the predictive value of a mature Amniostat-FLM result was 96.2 % , whereas that of an immature result was 58.5 % .
	manualset3
205704	6	417742	7	NULL	NULL	0	NULL	immature result	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With lecithin phosphorus concentration as the reference standard , the predictive value of a mature Amniostat-FLM result was 96.2 % , whereas that of an immature result was 58.5 % .
	manualset3
205705	7	417742	7	NULL	NULL	0	NULL	 58.5 %	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With lecithin phosphorus concentration as the reference standard , the predictive value of a mature Amniostat-FLM result was 96.2 % , whereas that of an immature result was 58.5 % .
	manualset3
205706	1	417743	7	NULL	NULL	0	NULL	phosphorylated H2B histone	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	With phosphorylated H2B histone as substrate , these effectors caused an increase in both Km and V values of the two forms of the enzyme .
	manualset3
205707	2	417743	7	NULL	NULL	0	NULL	substrate	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	With phosphorylated H2B histone as substrate , these effectors caused an increase in both Km and V values of the two forms of the enzyme .
	manualset3
205708	3	417743	7	NULL	NULL	0	NULL	effectors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	With phosphorylated H2B histone as substrate , these effectors caused an increase in both Km and V values of the two forms of the enzyme .
	manualset3
205709	4	417743	7	NULL	NULL	0	NULL	Km values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With phosphorylated H2B histone as substrate , these effectors caused an increase in both Km and V values of the two forms of the enzyme .
	manualset3
205710	5	417743	7	NULL	NULL	0	NULL	V values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With phosphorylated H2B histone as substrate , these effectors caused an increase in both Km and V values of the two forms of the enzyme .
	manualset3
205711	6	417743	7	NULL	NULL	0	NULL	two forms	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	With phosphorylated H2B histone as substrate , these effectors caused an increase in both Km and V values of the two forms of the enzyme .
	manualset3
205712	7	417743	7	NULL	NULL	0	NULL	enzyme	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	With phosphorylated H2B histone as substrate , these effectors caused an increase in both Km and V values of the two forms of the enzyme .
	manualset3
205713	1	417744	7	NULL	NULL	0	NULL	phytochemicals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	With phytochemicals executing a plethora of anti-tumor mechanisms , targeting the ` guardian angel ' p53 appears to be a critical strategy to energize the process of cancer therapeutics .
	manualset3
205714	2	417744	7	NULL	NULL	0	NULL	anti-tumor mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	With phytochemicals executing a plethora of anti-tumor mechanisms , targeting the ` guardian angel ' p53 appears to be a critical strategy to energize the process of cancer therapeutics .
	manualset3
205715	3	417744	7	NULL	NULL	0	NULL	 ` guardian angel ' p53	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	With phytochemicals executing a plethora of anti-tumor mechanisms , targeting the ` guardian angel ' p53 appears to be a critical strategy to energize the process of cancer therapeutics .
	manualset3
205716	4	417744	7	NULL	NULL	0	NULL	critical strategy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With phytochemicals executing a plethora of anti-tumor mechanisms , targeting the ` guardian angel ' p53 appears to be a critical strategy to energize the process of cancer therapeutics .
	manualset3
205717	5	417744	7	NULL	NULL	0	NULL	process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With phytochemicals executing a plethora of anti-tumor mechanisms , targeting the ` guardian angel ' p53 appears to be a critical strategy to energize the process of cancer therapeutics .
	manualset3
205718	6	417744	7	NULL	NULL	0	NULL	cancer therapeutics	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	With phytochemicals executing a plethora of anti-tumor mechanisms , targeting the ` guardian angel ' p53 appears to be a critical strategy to energize the process of cancer therapeutics .
	manualset3
205719	7	417744	7	NULL	NULL	0	NULL	targeting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With phytochemicals executing a plethora of anti-tumor mechanisms , targeting the ` guardian angel ' p53 appears to be a critical strategy to energize the process of cancer therapeutics .
	manualset3
205720	1	417745	7	NULL	NULL	0	NULL	polyacrylamide gel electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	With polyacrylamide gel electrophoresis in the presence of dodecyl sulphate , subunits with a molecular weight of 34 000 and higher aggregates of this size could be detected .
	manualset3
205721	2	417745	7	NULL	NULL	0	NULL	dodecyl sulphate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	With polyacrylamide gel electrophoresis in the presence of dodecyl sulphate , subunits with a molecular weight of 34 000 and higher aggregates of this size could be detected .
	manualset3
205722	3	417745	7	NULL	NULL	0	NULL	 subunits	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	With polyacrylamide gel electrophoresis in the presence of dodecyl sulphate , subunits with a molecular weight of 34 000 and higher aggregates of this size could be detected .
	manualset3
205723	4	417745	7	NULL	NULL	0	NULL	 molecular weight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With polyacrylamide gel electrophoresis in the presence of dodecyl sulphate , subunits with a molecular weight of 34 000 and higher aggregates of this size could be detected .
	manualset3
205724	5	417745	7	NULL	NULL	0	NULL	34 000	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	With polyacrylamide gel electrophoresis in the presence of dodecyl sulphate , subunits with a molecular weight of 34 000 and higher aggregates of this size could be detected .
	manualset3
205725	6	417745	7	NULL	NULL	0	NULL	higher aggregates	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	With polyacrylamide gel electrophoresis in the presence of dodecyl sulphate , subunits with a molecular weight of 34 000 and higher aggregates of this size could be detected .
	manualset3
205726	7	417745	7	NULL	NULL	0	NULL	size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With polyacrylamide gel electrophoresis in the presence of dodecyl sulphate , subunits with a molecular weight of 34 000 and higher aggregates of this size could be detected .
	manualset3
205727	1	417746	7	NULL	NULL	0	NULL	 pre -treatment samples	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	All pre - and posttreatment samples as well as gametocytes harbored a single copy of the Pfmdr1 gene and the wild-type allele ( L89 ) at codon 89 of the PfATPase6 gene .
	manualset3
205728	2	417746	7	NULL	NULL	0	NULL	posttreatment samples	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	All pre - and posttreatment samples as well as gametocytes harbored a single copy of the Pfmdr1 gene and the wild-type allele ( L89 ) at codon 89 of the PfATPase6 gene .
	manualset3
205729	3	417746	7	NULL	NULL	0	NULL	gametocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	All pre - and posttreatment samples as well as gametocytes harbored a single copy of the Pfmdr1 gene and the wild-type allele ( L89 ) at codon 89 of the PfATPase6 gene .
	manualset3
205730	4	417746	7	NULL	NULL	0	NULL	single copy	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	All pre - and posttreatment samples as well as gametocytes harbored a single copy of the Pfmdr1 gene and the wild-type allele ( L89 ) at codon 89 of the PfATPase6 gene .
	manualset3
205731	5	417746	7	NULL	NULL	0	NULL	Pfmdr1 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	All pre - and posttreatment samples as well as gametocytes harbored a single copy of the Pfmdr1 gene and the wild-type allele ( L89 ) at codon 89 of the PfATPase6 gene .
	manualset3
205732	6	417746	7	NULL	NULL	0	NULL	wild-type allele ( L89 )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	All pre - and posttreatment samples as well as gametocytes harbored a single copy of the Pfmdr1 gene and the wild-type allele ( L89 ) at codon 89 of the PfATPase6 gene .
	manualset3
205733	7	417746	7	NULL	NULL	0	NULL	codon 89	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	All pre - and posttreatment samples as well as gametocytes harbored a single copy of the Pfmdr1 gene and the wild-type allele ( L89 ) at codon 89 of the PfATPase6 gene .
	manualset3
205734	8	417746	7	NULL	NULL	0	NULL	PfATPase6 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	All pre - and posttreatment samples as well as gametocytes harbored a single copy of the Pfmdr1 gene and the wild-type allele ( L89 ) at codon 89 of the PfATPase6 gene .
	manualset3
205735	1	417747	7	NULL	NULL	NULL	NULL	recent developments	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	With recent developments in surgical techniques , the number of neorectal reservoir configurations has increased .
	manualset3
205736	2	417747	7	NULL	NULL	0	NULL	surgical techniques	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	With recent developments in surgical techniques , the number of neorectal reservoir configurations has increased .
	manualset3
205737	3	417747	7	NULL	NULL	0	NULL	 number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With recent developments in surgical techniques , the number of neorectal reservoir configurations has increased .
	manualset3
205738	4	417747	7	NULL	NULL	0	NULL	neorectal reservoir configurations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With recent developments in surgical techniques , the number of neorectal reservoir configurations has increased .
	manualset3
205739	1	417748	7	NULL	NULL	0	NULL	influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With regard to the influence of chemical composition , a striking example is provided by the suberic acid dye which gives particularly strong precipitin reactions , most probably on account of its long aliphatic side chains .
	manualset3
205740	2	417748	7	NULL	NULL	0	NULL	chemical composition	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With regard to the influence of chemical composition , a striking example is provided by the suberic acid dye which gives particularly strong precipitin reactions , most probably on account of its long aliphatic side chains .
	manualset3
205741	3	417748	7	NULL	NULL	0	NULL	example	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	With regard to the influence of chemical composition , a striking example is provided by the suberic acid dye which gives particularly strong precipitin reactions , most probably on account of its long aliphatic side chains .
	manualset3
205742	4	417748	7	NULL	NULL	0	NULL	suberic acid dye	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	With regard to the influence of chemical composition , a striking example is provided by the suberic acid dye which gives particularly strong precipitin reactions , most probably on account of its long aliphatic side chains .
	manualset3
205743	5	417748	7	NULL	NULL	0	NULL	strong precipitin reactions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With regard to the influence of chemical composition , a striking example is provided by the suberic acid dye which gives particularly strong precipitin reactions , most probably on account of its long aliphatic side chains .
	manualset3
205744	6	417748	7	NULL	NULL	0	NULL	long aliphatic side chains	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	With regard to the influence of chemical composition , a striking example is provided by the suberic acid dye which gives particularly strong precipitin reactions , most probably on account of its long aliphatic side chains .
	manualset3
205745	1	417749	7	NULL	NULL	0	NULL	working mechanism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With regard to the working mechanism the opinion is held that the immunological complex which is existant in the psoriatic epidermis participates to a great extent in the release of the epidermopoesis which is typical for the psoriasis .
	manualset3
205746	2	417749	7	NULL	NULL	0	NULL	opinion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With regard to the working mechanism the opinion is held that the immunological complex which is existant in the psoriatic epidermis participates to a great extent in the release of the epidermopoesis which is typical for the psoriasis .
	manualset3
205747	3	417749	7	NULL	NULL	NULL	NULL	immunological complex	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	With regard to the working mechanism the opinion is held that the immunological complex which is existant in the psoriatic epidermis participates to a great extent in the release of the epidermopoesis which is typical for the psoriasis .
	manualset3
205748	4	417749	7	NULL	NULL	NULL	NULL	psoriatic epidermis	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	With regard to the working mechanism the opinion is held that the immunological complex which is existant in the psoriatic epidermis participates to a great extent in the release of the epidermopoesis which is typical for the psoriasis .
	manualset3
205749	5	417749	7	NULL	NULL	0	NULL	great extent	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With regard to the working mechanism the opinion is held that the immunological complex which is existant in the psoriatic epidermis participates to a great extent in the release of the epidermopoesis which is typical for the psoriasis .
	manualset3
205750	6	417749	7	NULL	NULL	0	NULL	release	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With regard to the working mechanism the opinion is held that the immunological complex which is existant in the psoriatic epidermis participates to a great extent in the release of the epidermopoesis which is typical for the psoriasis .
	manualset3
205751	7	417749	7	NULL	NULL	0	NULL	epidermopoesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	With regard to the working mechanism the opinion is held that the immunological complex which is existant in the psoriatic epidermis participates to a great extent in the release of the epidermopoesis which is typical for the psoriasis .
	manualset3
205752	8	417749	7	NULL	NULL	0	NULL	psoriasis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	With regard to the working mechanism the opinion is held that the immunological complex which is existant in the psoriatic epidermis participates to a great extent in the release of the epidermopoesis which is typical for the psoriasis .
	manualset3
205753	1	417750	7	NULL	NULL	0	NULL	 36 Latin American countries	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	With regard to this point , 36 Latin American and Caribean countries will have an average life expectancy of 65 years , and 19 of 70 years .
	manualset3
205754	2	417750	7	NULL	NULL	0	NULL	Caribean countries 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	With regard to this point , 36 Latin American and Caribean countries will have an average life expectancy of 65 years , and 19 of 70 years .
	manualset3
205755	3	417750	7	NULL	NULL	NULL	NULL	average life expectancy	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	With regard to this point , 36 Latin American and Caribean countries will have an average life expectancy of 65 years , and 19 of 70 years .
	manualset3
205756	4	417750	7	NULL	NULL	0	NULL	65 years	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	With regard to this point , 36 Latin American and Caribean countries will have an average life expectancy of 65 years , and 19 of 70 years .
	manualset3
205757	5	417750	7	NULL	NULL	0	NULL	19 of 70 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	With regard to this point , 36 Latin American and Caribean countries will have an average life expectancy of 65 years , and 19 of 70 years .
	manualset3
207903	6	417750	7	NULL	NULL	0	NULL	point	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With regard to this point , 36 Latin American and Caribean countries will have an average life expectancy of 65 years , and 19 of 70 years .
	manualset3
205758	1	417751	7	NULL	NULL	0	NULL	local effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With respect to local effects , skin thickness and dermal DNA synthesis both proved to be good parameters .
	manualset3
205759	2	417751	7	NULL	NULL	0	NULL	skin thickness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With respect to local effects , skin thickness and dermal DNA synthesis both proved to be good parameters .
	manualset3
205760	3	417751	7	NULL	NULL	0	NULL	 dermal DNA synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	With respect to local effects , skin thickness and dermal DNA synthesis both proved to be good parameters .
	manualset3
205761	4	417751	7	NULL	NULL	0	NULL	good parameters	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With respect to local effects , skin thickness and dermal DNA synthesis both proved to be good parameters .
	manualset3
205762	1	417752	7	NULL	NULL	0	NULL	ulcerogenic properties	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With respect to their ulcerogenic properties , the formulations were significantly less active than IND alone , suggesting that a reduction in the ulcerogenic activity of IND was by produced complexation with egg albumin .
	manualset3
205763	2	417752	7	NULL	NULL	0	NULL	formulations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With respect to their ulcerogenic properties , the formulations were significantly less active than IND alone , suggesting that a reduction in the ulcerogenic activity of IND was by produced complexation with egg albumin .
	manualset3
205764	3	417752	7	NULL	NULL	0	NULL	IND	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	With respect to their ulcerogenic properties , the formulations were significantly less active than IND alone , suggesting that a reduction in the ulcerogenic activity of IND was by produced complexation with egg albumin .
	manualset3
205765	4	417752	7	NULL	NULL	0	NULL	 reduction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With respect to their ulcerogenic properties , the formulations were significantly less active than IND alone , suggesting that a reduction in the ulcerogenic activity of IND was by produced complexation with egg albumin .
	manualset3
205766	5	417752	7	NULL	NULL	0	NULL	ulcerogenic activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With respect to their ulcerogenic properties , the formulations were significantly less active than IND alone , suggesting that a reduction in the ulcerogenic activity of IND was by produced complexation with egg albumin .
	manualset3
205767	6	417752	7	NULL	NULL	0	NULL	IND	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	With respect to their ulcerogenic properties , the formulations were significantly less active than IND alone , suggesting that a reduction in the ulcerogenic activity of IND was by produced complexation with egg albumin .
	manualset3
205768	7	417752	7	NULL	NULL	0	NULL	complexation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With respect to their ulcerogenic properties , the formulations were significantly less active than IND alone , suggesting that a reduction in the ulcerogenic activity of IND was by produced complexation with egg albumin .
	manualset3
205769	8	417752	7	NULL	NULL	0	NULL	egg albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	With respect to their ulcerogenic properties , the formulations were significantly less active than IND alone , suggesting that a reduction in the ulcerogenic activity of IND was by produced complexation with egg albumin .
	manualset3
205770	1	417753	7	NULL	NULL	0	NULL	hypoxia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With reversal of hypoxia , Qp and ET-1 levels returned to baseline .
	manualset3
205771	2	417753	7	NULL	NULL	0	NULL	Qp levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With reversal of hypoxia , Qp and ET-1 levels returned to baseline .
	manualset3
205772	3	417753	7	NULL	NULL	0	NULL	ET-1 levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With reversal of hypoxia , Qp and ET-1 levels returned to baseline .
	manualset3
205773	4	417753	7	NULL	NULL	0	NULL	 baseline	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With reversal of hypoxia , Qp and ET-1 levels returned to baseline .
	manualset3
207904	5	417753	7	NULL	NULL	0	NULL	reversal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With reversal of hypoxia , Qp and ET-1 levels returned to baseline .
	manualset3
205774	1	417754	7	NULL	NULL	0	NULL	rabbits	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	All rabbits showed a reduction in the number of histochemically detectable stromal nerve trunks in the operated region .
	manualset3
205775	2	417754	7	NULL	NULL	0	NULL	 reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	All rabbits showed a reduction in the number of histochemically detectable stromal nerve trunks in the operated region .
	manualset3
205776	3	417754	7	NULL	NULL	0	NULL	 number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All rabbits showed a reduction in the number of histochemically detectable stromal nerve trunks in the operated region .
	manualset3
205778	4	417754	7	NULL	NULL	0	NULL	histochemically detectable stromal nerve trunks	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	All rabbits showed a reduction in the number of histochemically detectable stromal nerve trunks in the operated region .
	manualset3
205779	5	417754	7	NULL	NULL	0	NULL	operated region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	All rabbits showed a reduction in the number of histochemically detectable stromal nerve trunks in the operated region .
	manualset3
205782	1	417755	7	NULL	NULL	0	NULL	special reference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With special reference to the problem of nomenclature ) .
	manualset3
205783	2	417755	7	NULL	NULL	NULL	NULL	 problem 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	With special reference to the problem of nomenclature ) .
	manualset3
205784	3	417755	7	NULL	NULL	0	NULL	nomenclature	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	With special reference to the problem of nomenclature ) .
	manualset3
205787	1	417756	7	NULL	NULL	0	NULL	telemedical concepts	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	With telemedical concepts , continuous monitoring of the health status can be ensured , and consequently therapy management can be adapted to the individual requirements of every individual patient .
	manualset3
205788	2	417756	7	NULL	NULL	0	NULL	continuous monitoring	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	With telemedical concepts , continuous monitoring of the health status can be ensured , and consequently therapy management can be adapted to the individual requirements of every individual patient .
	manualset3
205789	3	417756	7	NULL	NULL	0	NULL	health status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With telemedical concepts , continuous monitoring of the health status can be ensured , and consequently therapy management can be adapted to the individual requirements of every individual patient .
	manualset3
205794	4	417756	7	NULL	NULL	0	NULL	therapy management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With telemedical concepts , continuous monitoring of the health status can be ensured , and consequently therapy management can be adapted to the individual requirements of every individual patient .
	manualset3
205796	5	417756	7	NULL	NULL	0	NULL	individual requirements 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With telemedical concepts , continuous monitoring of the health status can be ensured , and consequently therapy management can be adapted to the individual requirements of every individual patient .
	manualset3
205797	6	417756	7	NULL	NULL	0	NULL	individual patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	With telemedical concepts , continuous monitoring of the health status can be ensured , and consequently therapy management can be adapted to the individual requirements of every individual patient .
	manualset3
205798	1	417757	7	NULL	NULL	0	NULL	testosterone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	With testosterone as substrate , in the presence of LH and insulin , aromatase activity was stimulated up to 136 % , and in the presence of FSH and insulin , up to 156 % .
	manualset3
205799	2	417757	7	NULL	NULL	0	NULL	substrate	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	With testosterone as substrate , in the presence of LH and insulin , aromatase activity was stimulated up to 136 % , and in the presence of FSH and insulin , up to 156 % .
	manualset3
205801	3	417757	7	NULL	NULL	0	NULL	LH	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	With testosterone as substrate , in the presence of LH and insulin , aromatase activity was stimulated up to 136 % , and in the presence of FSH and insulin , up to 156 % .
	manualset3
205803	4	417757	7	NULL	NULL	0	NULL	insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	With testosterone as substrate , in the presence of LH and insulin , aromatase activity was stimulated up to 136 % , and in the presence of FSH and insulin , up to 156 % .
	manualset3
205805	5	417757	7	NULL	NULL	0	NULL	aromatase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	With testosterone as substrate , in the presence of LH and insulin , aromatase activity was stimulated up to 136 % , and in the presence of FSH and insulin , up to 156 % .
	manualset3
205806	6	417757	7	NULL	NULL	0	NULL	136 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With testosterone as substrate , in the presence of LH and insulin , aromatase activity was stimulated up to 136 % , and in the presence of FSH and insulin , up to 156 % .
	manualset3
205807	7	417757	7	NULL	NULL	0	NULL	FSH	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	With testosterone as substrate , in the presence of LH and insulin , aromatase activity was stimulated up to 136 % , and in the presence of FSH and insulin , up to 156 % .
	manualset3
205808	8	417757	7	NULL	NULL	0	NULL	insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	With testosterone as substrate , in the presence of LH and insulin , aromatase activity was stimulated up to 136 % , and in the presence of FSH and insulin , up to 156 % .
	manualset3
205809	9	417757	7	NULL	NULL	0	NULL	156 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With testosterone as substrate , in the presence of LH and insulin , aromatase activity was stimulated up to 136 % , and in the presence of FSH and insulin , up to 156 % .
	manualset3
205874	1	417758	7	NULL	NULL	0	NULL	 IIF	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	With the IIF using mAb C6 , oocysts appeared as 3 to 5 microns spherical objects fluorescing bright apple green against a reddish dark background .
	manualset3
205875	2	417758	7	NULL	NULL	0	NULL	mAb C6 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	With the IIF using mAb C6 , oocysts appeared as 3 to 5 microns spherical objects fluorescing bright apple green against a reddish dark background .
	manualset3
205876	3	417758	7	NULL	NULL	0	NULL	 oocysts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	With the IIF using mAb C6 , oocysts appeared as 3 to 5 microns spherical objects fluorescing bright apple green against a reddish dark background .
	manualset3
205877	4	417758	7	NULL	NULL	0	NULL	 3 to 5 microns	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With the IIF using mAb C6 , oocysts appeared as 3 to 5 microns spherical objects fluorescing bright apple green against a reddish dark background .
	manualset3
205878	5	417758	7	NULL	NULL	NULL	NULL	spherical objects fluorescing bright apple green against a reddish dark background	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	With the IIF using mAb C6 , oocysts appeared as 3 to 5 microns spherical objects fluorescing bright apple green against a reddish dark background .
	manualset3
205880	1	417759	7	NULL	NULL	0	NULL	advantage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the advantage of the complete RFLP pattern available from CE , it appears to be more convenient to use an electropherogram rather than performing the cumbersome slab gel electrophoresis plus diagnostic algorithm to identify Mycobacterium species .
	manualset3
205881	2	417759	7	NULL	NULL	0	NULL	complete RFLP pattern	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the advantage of the complete RFLP pattern available from CE , it appears to be more convenient to use an electropherogram rather than performing the cumbersome slab gel electrophoresis plus diagnostic algorithm to identify Mycobacterium species .
	manualset3
205882	3	417759	7	NULL	NULL	0	NULL	CE	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	With the advantage of the complete RFLP pattern available from CE , it appears to be more convenient to use an electropherogram rather than performing the cumbersome slab gel electrophoresis plus diagnostic algorithm to identify Mycobacterium species .
	manualset3
205883	4	417759	7	NULL	NULL	0	NULL	electropherogram	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	With the advantage of the complete RFLP pattern available from CE , it appears to be more convenient to use an electropherogram rather than performing the cumbersome slab gel electrophoresis plus diagnostic algorithm to identify Mycobacterium species .
	manualset3
205884	5	417759	7	NULL	NULL	0	NULL	slab gel electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	With the advantage of the complete RFLP pattern available from CE , it appears to be more convenient to use an electropherogram rather than performing the cumbersome slab gel electrophoresis plus diagnostic algorithm to identify Mycobacterium species .
	manualset3
205885	6	417759	7	NULL	NULL	0	NULL	diagnostic algorithm	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	With the advantage of the complete RFLP pattern available from CE , it appears to be more convenient to use an electropherogram rather than performing the cumbersome slab gel electrophoresis plus diagnostic algorithm to identify Mycobacterium species .
	manualset3
205886	7	417759	7	NULL	NULL	0	NULL	Mycobacterium species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	With the advantage of the complete RFLP pattern available from CE , it appears to be more convenient to use an electropherogram rather than performing the cumbersome slab gel electrophoresis plus diagnostic algorithm to identify Mycobacterium species .
	manualset3
205887	1	417760	7	NULL	NULL	0	NULL	advent	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the advent of recombinant DNA methodologies combined with site-directed mutagenesis , a variety of structural modifications becomes possible .
	manualset3
205888	2	417760	7	NULL	NULL	0	NULL	recombinant DNA methodologies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	With the advent of recombinant DNA methodologies combined with site-directed mutagenesis , a variety of structural modifications becomes possible .
	manualset3
205889	3	417760	7	NULL	NULL	0	NULL	site-directed mutagenesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	With the advent of recombinant DNA methodologies combined with site-directed mutagenesis , a variety of structural modifications becomes possible .
	manualset3
205891	4	417760	7	NULL	NULL	NULL	NULL	structural modifications	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	With the advent of recombinant DNA methodologies combined with site-directed mutagenesis , a variety of structural modifications becomes possible .
	manualset3
205895	5	417760	7	NULL	NULL	0	NULL	variety	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	With the advent of recombinant DNA methodologies combined with site-directed mutagenesis , a variety of structural modifications becomes possible .
	manualset3
205896	1	417761	7	NULL	NULL	NULL	NULL	  caveats 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	With the caveats of viral vector-based therapeutics largely centered on a lack of in vivo control , the recent success of exploiting microRNA expression to limit viral tropism may breathe new life into the field .
	manualset3
205897	2	417761	7	NULL	NULL	0	NULL	viral vector-based therapeutics	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	With the caveats of viral vector-based therapeutics largely centered on a lack of in vivo control , the recent success of exploiting microRNA expression to limit viral tropism may breathe new life into the field .
	manualset3
205899	3	417761	7	NULL	NULL	NULL	NULL	 recent success	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	With the caveats of viral vector-based therapeutics largely centered on a lack of in vivo control , the recent success of exploiting microRNA expression to limit viral tropism may breathe new life into the field .
	manualset3
205901	4	417761	7	NULL	NULL	0	NULL	microRNA expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	With the caveats of viral vector-based therapeutics largely centered on a lack of in vivo control , the recent success of exploiting microRNA expression to limit viral tropism may breathe new life into the field .
	manualset3
205903	5	417761	7	NULL	NULL	0	NULL	viral tropism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	With the caveats of viral vector-based therapeutics largely centered on a lack of in vivo control , the recent success of exploiting microRNA expression to limit viral tropism may breathe new life into the field .
	manualset3
205906	6	417761	7	NULL	NULL	0	NULL	new life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	With the caveats of viral vector-based therapeutics largely centered on a lack of in vivo control , the recent success of exploiting microRNA expression to limit viral tropism may breathe new life into the field .
	manualset3
205907	7	417761	7	NULL	NULL	0	NULL	field	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	With the caveats of viral vector-based therapeutics largely centered on a lack of in vivo control , the recent success of exploiting microRNA expression to limit viral tropism may breathe new life into the field .
	manualset3
207905	8	417761	7	NULL	NULL	0	NULL	lack	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the caveats of viral vector-based therapeutics largely centered on a lack of in vivo control , the recent success of exploiting microRNA expression to limit viral tropism may breathe new life into the field .
	manualset3
207906	9	417761	7	NULL	NULL	0	NULL	 in vivo control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the caveats of viral vector-based therapeutics largely centered on a lack of in vivo control , the recent success of exploiting microRNA expression to limit viral tropism may breathe new life into the field .
	manualset3
205919	1	417762	7	NULL	NULL	0	NULL	emergence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the emergence of new , effective targeted molecular therapies for mRCC , well-designed prospective trials are needed to clarify the biologic effects of CN to determine when and for whom CN should be performed in the context of targeted systemic therapy .
	manualset3
205920	2	417762	7	NULL	NULL	0	NULL	targeted molecular therapies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	With the emergence of new , effective targeted molecular therapies for mRCC , well-designed prospective trials are needed to clarify the biologic effects of CN to determine when and for whom CN should be performed in the context of targeted systemic therapy .
	manualset3
205921	3	417762	7	NULL	NULL	0	NULL	mRCC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	With the emergence of new , effective targeted molecular therapies for mRCC , well-designed prospective trials are needed to clarify the biologic effects of CN to determine when and for whom CN should be performed in the context of targeted systemic therapy .
	manualset3
205922	4	417762	7	NULL	NULL	0	NULL	 prospective trials 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	With the emergence of new , effective targeted molecular therapies for mRCC , well-designed prospective trials are needed to clarify the biologic effects of CN to determine when and for whom CN should be performed in the context of targeted systemic therapy .
	manualset3
205923	5	417762	7	NULL	NULL	0	NULL	 biologic effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the emergence of new , effective targeted molecular therapies for mRCC , well-designed prospective trials are needed to clarify the biologic effects of CN to determine when and for whom CN should be performed in the context of targeted systemic therapy .
	manualset3
205924	6	417762	7	NULL	NULL	0	NULL	CN	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	With the emergence of new , effective targeted molecular therapies for mRCC , well-designed prospective trials are needed to clarify the biologic effects of CN to determine when and for whom CN should be performed in the context of targeted systemic therapy .
	manualset3
205925	7	417762	7	NULL	NULL	0	NULL	CN	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	With the emergence of new , effective targeted molecular therapies for mRCC , well-designed prospective trials are needed to clarify the biologic effects of CN to determine when and for whom CN should be performed in the context of targeted systemic therapy .
	manualset3
205926	8	417762	7	NULL	NULL	0	NULL	context 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the emergence of new , effective targeted molecular therapies for mRCC , well-designed prospective trials are needed to clarify the biologic effects of CN to determine when and for whom CN should be performed in the context of targeted systemic therapy .
	manualset3
205927	9	417762	7	NULL	NULL	0	NULL	targeted systemic therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	With the emergence of new , effective targeted molecular therapies for mRCC , well-designed prospective trials are needed to clarify the biologic effects of CN to determine when and for whom CN should be performed in the context of targeted systemic therapy .
	manualset3
205937	1	417763	7	NULL	NULL	0	NULL	exception	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the exception of a very high A+T - content and the presence of multiple repetitions , no general rule at the basis of this phenomenon is actually known .
	manualset3
205938	2	417763	7	NULL	NULL	0	NULL	high A+T - content 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With the exception of a very high A+T - content and the presence of multiple repetitions , no general rule at the basis of this phenomenon is actually known .
	manualset3
205939	3	417763	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the exception of a very high A+T - content and the presence of multiple repetitions , no general rule at the basis of this phenomenon is actually known .
	manualset3
205940	4	417763	7	NULL	NULL	0	NULL	multiple repetitions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the exception of a very high A+T - content and the presence of multiple repetitions , no general rule at the basis of this phenomenon is actually known .
	manualset3
205941	5	417763	7	NULL	NULL	0	NULL	general rule	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the exception of a very high A+T - content and the presence of multiple repetitions , no general rule at the basis of this phenomenon is actually known .
	manualset3
205942	6	417763	7	NULL	NULL	0	NULL	basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the exception of a very high A+T - content and the presence of multiple repetitions , no general rule at the basis of this phenomenon is actually known .
	manualset3
205943	7	417763	7	NULL	NULL	0	NULL	phenomenon 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the exception of a very high A+T - content and the presence of multiple repetitions , no general rule at the basis of this phenomenon is actually known .
	manualset3
205993	1	417764	7	NULL	NULL	0	NULL	 exception	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With the exception of peribronchial glands and chondrocytes of peribronchial cartilage , COX-2 is not detectable in the normal lung of nonhuman primates .
	manualset3
205994	2	417764	7	NULL	NULL	0	NULL	peribronchial glands	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	With the exception of peribronchial glands and chondrocytes of peribronchial cartilage , COX-2 is not detectable in the normal lung of nonhuman primates .
	manualset3
205995	3	417764	7	NULL	NULL	0	NULL	chondrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	With the exception of peribronchial glands and chondrocytes of peribronchial cartilage , COX-2 is not detectable in the normal lung of nonhuman primates .
	manualset3
205996	4	417764	7	NULL	NULL	0	NULL	peribronchial cartilage	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	With the exception of peribronchial glands and chondrocytes of peribronchial cartilage , COX-2 is not detectable in the normal lung of nonhuman primates .
	manualset3
205997	5	417764	7	NULL	NULL	0	NULL	COX-2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	With the exception of peribronchial glands and chondrocytes of peribronchial cartilage , COX-2 is not detectable in the normal lung of nonhuman primates .
	manualset3
205998	6	417764	7	NULL	NULL	0	NULL	 lung 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	With the exception of peribronchial glands and chondrocytes of peribronchial cartilage , COX-2 is not detectable in the normal lung of nonhuman primates .
	manualset3
205999	7	417764	7	NULL	NULL	0	NULL	 nonhuman primates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	With the exception of peribronchial glands and chondrocytes of peribronchial cartilage , COX-2 is not detectable in the normal lung of nonhuman primates .
	manualset3
206000	1	417765	7	NULL	NULL	0	NULL	growing number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With the growing number of available certifications , college students are expected to have a college degree and obtain multiple fitness related certifications before being considered for a personal training position .
	manualset3
206001	2	417765	7	NULL	NULL	NULL	NULL	 certifications 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	With the growing number of available certifications , college students are expected to have a college degree and obtain multiple fitness related certifications before being considered for a personal training position .
	manualset3
206002	3	417765	7	NULL	NULL	0	NULL	college students	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	With the growing number of available certifications , college students are expected to have a college degree and obtain multiple fitness related certifications before being considered for a personal training position .
	manualset3
206003	4	417765	7	NULL	NULL	0	NULL	college degree	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	With the growing number of available certifications , college students are expected to have a college degree and obtain multiple fitness related certifications before being considered for a personal training position .
	manualset3
206004	5	417765	7	NULL	NULL	0	NULL	multiple fitness related certifications	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	With the growing number of available certifications , college students are expected to have a college degree and obtain multiple fitness related certifications before being considered for a personal training position .
	manualset3
206005	6	417765	7	NULL	NULL	0	NULL	personal training position	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the growing number of available certifications , college students are expected to have a college degree and obtain multiple fitness related certifications before being considered for a personal training position .
	manualset3
206006	1	417766	7	NULL	NULL	0	NULL	growing popularity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the growing popularity of recreational scuba diving , emergency physicians are liable to be faced with increasing numbers of diving-related medical problems .
	manualset3
206007	2	417766	7	NULL	NULL	0	NULL	recreational scuba diving	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	With the growing popularity of recreational scuba diving , emergency physicians are liable to be faced with increasing numbers of diving-related medical problems .
	manualset3
206008	3	417766	7	NULL	NULL	0	NULL	emergency physicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	With the growing popularity of recreational scuba diving , emergency physicians are liable to be faced with increasing numbers of diving-related medical problems .
	manualset3
206009	4	417766	7	NULL	NULL	0	NULL	increasing numbers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With the growing popularity of recreational scuba diving , emergency physicians are liable to be faced with increasing numbers of diving-related medical problems .
	manualset3
206010	5	417766	7	NULL	NULL	0	NULL	diving-related medical problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With the growing popularity of recreational scuba diving , emergency physicians are liable to be faced with increasing numbers of diving-related medical problems .
	manualset3
206011	1	417767	7	NULL	NULL	0	NULL	help	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the help of this material , the bulb part is connected to the plate as a labile piece , and this connection acts like a natural velopharyngeal extension .
	manualset3
206012	2	417767	7	NULL	NULL	NULL	NULL	material	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	With the help of this material , the bulb part is connected to the plate as a labile piece , and this connection acts like a natural velopharyngeal extension .
	manualset3
206013	3	417767	7	NULL	NULL	0	NULL	bulb part	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	With the help of this material , the bulb part is connected to the plate as a labile piece , and this connection acts like a natural velopharyngeal extension .
	manualset3
206014	4	417767	7	NULL	NULL	0	NULL	plate 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	With the help of this material , the bulb part is connected to the plate as a labile piece , and this connection acts like a natural velopharyngeal extension .
	manualset3
206015	5	417767	7	NULL	NULL	0	NULL	labile piece 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	With the help of this material , the bulb part is connected to the plate as a labile piece , and this connection acts like a natural velopharyngeal extension .
	manualset3
206016	6	417767	7	NULL	NULL	0	NULL	 connection 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	With the help of this material , the bulb part is connected to the plate as a labile piece , and this connection acts like a natural velopharyngeal extension .
	manualset3
206017	7	417767	7	NULL	NULL	0	NULL	natural velopharyngeal extension	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	With the help of this material , the bulb part is connected to the plate as a labile piece , and this connection acts like a natural velopharyngeal extension .
	manualset3
206018	1	417768	7	NULL	NULL	0	NULL	hypothesis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	With the hypothesis that aquaporins ( AQPs ) might be present in the colon epithelium of O. degus and involved in fluid absorption , we studied colon water absorption in vivo and the distribution of AQPs and Na ( + ) transporters by immunocytochemistry .
	manualset3
206019	2	417768	7	NULL	NULL	NULL	NULL	aquaporins ( AQPs )	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	With the hypothesis that aquaporins ( AQPs ) might be present in the colon epithelium of O. degus and involved in fluid absorption , we studied colon water absorption in vivo and the distribution of AQPs and Na ( + ) transporters by immunocytochemistry .
	manualset3
206020	3	417768	7	NULL	NULL	0	NULL	colon epithelium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	With the hypothesis that aquaporins ( AQPs ) might be present in the colon epithelium of O. degus and involved in fluid absorption , we studied colon water absorption in vivo and the distribution of AQPs and Na ( + ) transporters by immunocytochemistry .
	manualset3
206021	4	417768	7	NULL	NULL	0	NULL	O. degus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	With the hypothesis that aquaporins ( AQPs ) might be present in the colon epithelium of O. degus and involved in fluid absorption , we studied colon water absorption in vivo and the distribution of AQPs and Na ( + ) transporters by immunocytochemistry .
	manualset3
206022	5	417768	7	NULL	NULL	0	NULL	fluid absorption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	With the hypothesis that aquaporins ( AQPs ) might be present in the colon epithelium of O. degus and involved in fluid absorption , we studied colon water absorption in vivo and the distribution of AQPs and Na ( + ) transporters by immunocytochemistry .
	manualset3
206023	6	417768	7	NULL	NULL	0	NULL	colon water absorption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	With the hypothesis that aquaporins ( AQPs ) might be present in the colon epithelium of O. degus and involved in fluid absorption , we studied colon water absorption in vivo and the distribution of AQPs and Na ( + ) transporters by immunocytochemistry .
	manualset3
206024	7	417768	7	NULL	NULL	0	NULL	distribution 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	With the hypothesis that aquaporins ( AQPs ) might be present in the colon epithelium of O. degus and involved in fluid absorption , we studied colon water absorption in vivo and the distribution of AQPs and Na ( + ) transporters by immunocytochemistry .
	manualset3
206025	8	417768	7	NULL	NULL	0	NULL	AQPs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	With the hypothesis that aquaporins ( AQPs ) might be present in the colon epithelium of O. degus and involved in fluid absorption , we studied colon water absorption in vivo and the distribution of AQPs and Na ( + ) transporters by immunocytochemistry .
	manualset3
206026	9	417768	7	NULL	NULL	0	NULL	Na ( + ) transporters	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	With the hypothesis that aquaporins ( AQPs ) might be present in the colon epithelium of O. degus and involved in fluid absorption , we studied colon water absorption in vivo and the distribution of AQPs and Na ( + ) transporters by immunocytochemistry .
	manualset3
206027	10	417768	7	NULL	NULL	0	NULL	immunocytochemistry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	With the hypothesis that aquaporins ( AQPs ) might be present in the colon epithelium of O. degus and involved in fluid absorption , we studied colon water absorption in vivo and the distribution of AQPs and Na ( + ) transporters by immunocytochemistry .
	manualset3
206028	1	417769	7	NULL	NULL	0	NULL	increasing number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With the increasing number of reports of Pseudomonas infections related to the use of hydrotherapy equipment , the importance for further investigation into burn wound care with and without hydrotherapy , infection rates , and cost analysis appears to be indicated .
	manualset3
206029	2	417769	7	NULL	NULL	0	NULL	reports	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	With the increasing number of reports of Pseudomonas infections related to the use of hydrotherapy equipment , the importance for further investigation into burn wound care with and without hydrotherapy , infection rates , and cost analysis appears to be indicated .
	manualset3
206030	3	417769	7	NULL	NULL	0	NULL	Pseudomonas infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With the increasing number of reports of Pseudomonas infections related to the use of hydrotherapy equipment , the importance for further investigation into burn wound care with and without hydrotherapy , infection rates , and cost analysis appears to be indicated .
	manualset3
206031	4	417769	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the increasing number of reports of Pseudomonas infections related to the use of hydrotherapy equipment , the importance for further investigation into burn wound care with and without hydrotherapy , infection rates , and cost analysis appears to be indicated .
	manualset3
206032	5	417769	7	NULL	NULL	0	NULL	hydrotherapy equipment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	With the increasing number of reports of Pseudomonas infections related to the use of hydrotherapy equipment , the importance for further investigation into burn wound care with and without hydrotherapy , infection rates , and cost analysis appears to be indicated .
	manualset3
206033	6	417769	7	NULL	NULL	0	NULL	investigation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	With the increasing number of reports of Pseudomonas infections related to the use of hydrotherapy equipment , the importance for further investigation into burn wound care with and without hydrotherapy , infection rates , and cost analysis appears to be indicated .
	manualset3
206034	7	417769	7	NULL	NULL	0	NULL	burn wound care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	With the increasing number of reports of Pseudomonas infections related to the use of hydrotherapy equipment , the importance for further investigation into burn wound care with and without hydrotherapy , infection rates , and cost analysis appears to be indicated .
	manualset3
206035	8	417769	7	NULL	NULL	0	NULL	hydrotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	With the increasing number of reports of Pseudomonas infections related to the use of hydrotherapy equipment , the importance for further investigation into burn wound care with and without hydrotherapy , infection rates , and cost analysis appears to be indicated .
	manualset3
206036	9	417769	7	NULL	NULL	0	NULL	infection rates	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With the increasing number of reports of Pseudomonas infections related to the use of hydrotherapy equipment , the importance for further investigation into burn wound care with and without hydrotherapy , infection rates , and cost analysis appears to be indicated .
	manualset3
206037	10	417769	7	NULL	NULL	0	NULL	cost analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	With the increasing number of reports of Pseudomonas infections related to the use of hydrotherapy equipment , the importance for further investigation into burn wound care with and without hydrotherapy , infection rates , and cost analysis appears to be indicated .
	manualset3
206038	1	417770	7	NULL	NULL	0	NULL	topological gold layer	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	With the introduced topological gold layer , the photocurrent and efficiency are increased by 16 % and 18 % , respectively , due to the increased light collection .
	manualset3
206039	2	417770	7	NULL	NULL	0	NULL	 photocurrent 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	With the introduced topological gold layer , the photocurrent and efficiency are increased by 16 % and 18 % , respectively , due to the increased light collection .
	manualset3
206040	3	417770	7	NULL	NULL	0	NULL	16 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With the introduced topological gold layer , the photocurrent and efficiency are increased by 16 % and 18 % , respectively , due to the increased light collection .
	manualset3
206041	4	417770	7	NULL	NULL	0	NULL	18 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With the introduced topological gold layer , the photocurrent and efficiency are increased by 16 % and 18 % , respectively , due to the increased light collection .
	manualset3
206042	5	417770	7	NULL	NULL	0	NULL	light collection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	With the introduced topological gold layer , the photocurrent and efficiency are increased by 16 % and 18 % , respectively , due to the increased light collection .
	manualset3
206043	6	417770	7	NULL	NULL	0	NULL	efficiency	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the introduced topological gold layer , the photocurrent and efficiency are increased by 16 % and 18 % , respectively , due to the increased light collection .
	manualset3
206044	1	417771	7	NULL	NULL	0	NULL	introduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the introduction of clinical governance , and the statutory duty of health organizations to provide a quality service for patients supported by evidence-based practice , this article discusses isolation practices .
	manualset3
206045	2	417771	7	NULL	NULL	0	NULL	clinical governance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the introduction of clinical governance , and the statutory duty of health organizations to provide a quality service for patients supported by evidence-based practice , this article discusses isolation practices .
	manualset3
206046	3	417771	7	NULL	NULL	0	NULL	statutory duty 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the introduction of clinical governance , and the statutory duty of health organizations to provide a quality service for patients supported by evidence-based practice , this article discusses isolation practices .
	manualset3
206047	4	417771	7	NULL	NULL	0	NULL	 health organizations	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	With the introduction of clinical governance , and the statutory duty of health organizations to provide a quality service for patients supported by evidence-based practice , this article discusses isolation practices .
	manualset3
206048	5	417771	7	NULL	NULL	0	NULL	quality service	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the introduction of clinical governance , and the statutory duty of health organizations to provide a quality service for patients supported by evidence-based practice , this article discusses isolation practices .
	manualset3
206049	6	417771	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	With the introduction of clinical governance , and the statutory duty of health organizations to provide a quality service for patients supported by evidence-based practice , this article discusses isolation practices .
	manualset3
206050	7	417771	7	NULL	NULL	0	NULL	 evidence-based practice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the introduction of clinical governance , and the statutory duty of health organizations to provide a quality service for patients supported by evidence-based practice , this article discusses isolation practices .
	manualset3
206051	8	417771	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	With the introduction of clinical governance , and the statutory duty of health organizations to provide a quality service for patients supported by evidence-based practice , this article discusses isolation practices .
	manualset3
206052	9	417771	7	NULL	NULL	0	NULL	isolation practices	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the introduction of clinical governance , and the statutory duty of health organizations to provide a quality service for patients supported by evidence-based practice , this article discusses isolation practices .
	manualset3
206053	1	417772	7	NULL	NULL	0	NULL	Course	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Course of the concentration of serum free amino acids as a function of time and the method of preservation ) .
	manualset3
206054	2	417772	7	NULL	NULL	0	NULL	 concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Course of the concentration of serum free amino acids as a function of time and the method of preservation ) .
	manualset3
206055	3	417772	7	NULL	NULL	0	NULL	serum free amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	( Course of the concentration of serum free amino acids as a function of time and the method of preservation ) .
	manualset3
206056	4	417772	7	NULL	NULL	0	NULL	function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Course of the concentration of serum free amino acids as a function of time and the method of preservation ) .
	manualset3
206057	5	417772	7	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	( Course of the concentration of serum free amino acids as a function of time and the method of preservation ) .
	manualset3
206058	6	417772	7	NULL	NULL	0	NULL	method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Course of the concentration of serum free amino acids as a function of time and the method of preservation ) .
	manualset3
206059	7	417772	7	NULL	NULL	0	NULL	preservation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Course of the concentration of serum free amino acids as a function of time and the method of preservation ) .
	manualset3
206060	1	417773	7	NULL	NULL	0	NULL	 recombinant viruses 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	All recombinant viruses tested in Spodoptera frugiperda ( SF21 ) cells expressed a protein of about 18 kD which comigrated in PAGE with ATF from infected plants .
	manualset3
206061	2	417773	7	NULL	NULL	0	NULL	Spodoptera frugiperda ( SF21 ) cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	All recombinant viruses tested in Spodoptera frugiperda ( SF21 ) cells expressed a protein of about 18 kD which comigrated in PAGE with ATF from infected plants .
	manualset3
206062	3	417773	7	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	All recombinant viruses tested in Spodoptera frugiperda ( SF21 ) cells expressed a protein of about 18 kD which comigrated in PAGE with ATF from infected plants .
	manualset3
206063	4	417773	7	NULL	NULL	0	NULL	18 kD	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All recombinant viruses tested in Spodoptera frugiperda ( SF21 ) cells expressed a protein of about 18 kD which comigrated in PAGE with ATF from infected plants .
	manualset3
206064	5	417773	7	NULL	NULL	0	NULL	 PAGE	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	All recombinant viruses tested in Spodoptera frugiperda ( SF21 ) cells expressed a protein of about 18 kD which comigrated in PAGE with ATF from infected plants .
	manualset3
206065	6	417773	7	NULL	NULL	0	NULL	ATF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	All recombinant viruses tested in Spodoptera frugiperda ( SF21 ) cells expressed a protein of about 18 kD which comigrated in PAGE with ATF from infected plants .
	manualset3
206066	7	417773	7	NULL	NULL	0	NULL	infected plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	All recombinant viruses tested in Spodoptera frugiperda ( SF21 ) cells expressed a protein of about 18 kD which comigrated in PAGE with ATF from infected plants .
	manualset3
206067	1	417774	7	NULL	NULL	0	NULL	 introduction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the introduction of monoclonal antibodies in cancer immunotherapy complement has come into play with a great potential as effector system .
	manualset3
206068	2	417774	7	NULL	NULL	0	NULL	monoclonal antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	With the introduction of monoclonal antibodies in cancer immunotherapy complement has come into play with a great potential as effector system .
	manualset3
206069	3	417774	7	NULL	NULL	NULL	NULL	 cancer immunotherapy 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	With the introduction of monoclonal antibodies in cancer immunotherapy complement has come into play with a great potential as effector system .
	manualset3
206070	5	417774	7	NULL	NULL	NULL	NULL	great potential 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	With the introduction of monoclonal antibodies in cancer immunotherapy complement has come into play with a great potential as effector system .
	manualset3
206071	4	417774	7	NULL	NULL	0	NULL	complement	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	With the introduction of monoclonal antibodies in cancer immunotherapy complement has come into play with a great potential as effector system .
	manualset3
206072	6	417774	7	NULL	NULL	NULL	NULL	effector system	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	With the introduction of monoclonal antibodies in cancer immunotherapy complement has come into play with a great potential as effector system .
	manualset3
206073	1	417775	7	NULL	NULL	0	NULL	progression	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the progression of cartilage degeneration ( increased Collins grades and OA ) OP-1 protein was down-regulated up to 9-fold .
	manualset3
206074	2	417775	7	NULL	NULL	0	NULL	 cartilage degeneration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With the progression of cartilage degeneration ( increased Collins grades and OA ) OP-1 protein was down-regulated up to 9-fold .
	manualset3
206075	3	417775	7	NULL	NULL	0	NULL	increased Collins grades 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With the progression of cartilage degeneration ( increased Collins grades and OA ) OP-1 protein was down-regulated up to 9-fold .
	manualset3
206076	4	417775	7	NULL	NULL	0	NULL	OA	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	With the progression of cartilage degeneration ( increased Collins grades and OA ) OP-1 protein was down-regulated up to 9-fold .
	manualset3
206077	5	417775	7	NULL	NULL	0	NULL	OP-1 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	With the progression of cartilage degeneration ( increased Collins grades and OA ) OP-1 protein was down-regulated up to 9-fold .
	manualset3
206078	6	417775	7	NULL	NULL	0	NULL	9-fold 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With the progression of cartilage degeneration ( increased Collins grades and OA ) OP-1 protein was down-regulated up to 9-fold .
	manualset3
206079	1	417776	7	NULL	NULL	0	NULL	composite controller	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	With the proposed composite controller , the percent-RMS errors at 1 Hz and 25 Hz are reduced to 0.035 % and 0.31 % , respectively .
	manualset3
206080	2	417776	7	NULL	NULL	0	NULL	percent-RMS errors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With the proposed composite controller , the percent-RMS errors at 1 Hz and 25 Hz are reduced to 0.035 % and 0.31 % , respectively .
	manualset3
206081	3	417776	7	NULL	NULL	0	NULL	1 Hz	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With the proposed composite controller , the percent-RMS errors at 1 Hz and 25 Hz are reduced to 0.035 % and 0.31 % , respectively .
	manualset3
206082	4	417776	7	NULL	NULL	0	NULL	25 Hz 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With the proposed composite controller , the percent-RMS errors at 1 Hz and 25 Hz are reduced to 0.035 % and 0.31 % , respectively .
	manualset3
206083	5	417776	7	NULL	NULL	0	NULL	0.035 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	With the proposed composite controller , the percent-RMS errors at 1 Hz and 25 Hz are reduced to 0.035 % and 0.31 % , respectively .
	manualset3
206084	6	417776	7	NULL	NULL	0	NULL	0.31 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	With the proposed composite controller , the percent-RMS errors at 1 Hz and 25 Hz are reduced to 0.035 % and 0.31 % , respectively .
	manualset3
206085	1	417777	7	NULL	NULL	0	NULL	scientific advancements	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	With the scientific advancements in the management of malignant diseases , the treatment is expensive and bears high morbidity in term of oral mucositis .
	manualset3
206086	2	417777	7	NULL	NULL	0	NULL	management 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the scientific advancements in the management of malignant diseases , the treatment is expensive and bears high morbidity in term of oral mucositis .
	manualset3
206087	3	417777	7	NULL	NULL	0	NULL	malignant diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	With the scientific advancements in the management of malignant diseases , the treatment is expensive and bears high morbidity in term of oral mucositis .
	manualset3
206088	4	417777	7	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	With the scientific advancements in the management of malignant diseases , the treatment is expensive and bears high morbidity in term of oral mucositis .
	manualset3
206089	5	417777	7	NULL	NULL	0	NULL	high morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With the scientific advancements in the management of malignant diseases , the treatment is expensive and bears high morbidity in term of oral mucositis .
	manualset3
206090	6	417777	7	NULL	NULL	0	NULL	oral mucositis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	With the scientific advancements in the management of malignant diseases , the treatment is expensive and bears high morbidity in term of oral mucositis .
	manualset3
206091	1	417778	7	NULL	NULL	0	NULL	vinyl boronates 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	With the vinyl boronates , the Zr-Csp2 bond is initially cleaved by 1 equiv of electrophile .
	manualset3
206092	2	417778	7	NULL	NULL	0	NULL	Zr-Csp2 bond	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	With the vinyl boronates , the Zr-Csp2 bond is initially cleaved by 1 equiv of electrophile .
	manualset3
206093	3	417778	7	NULL	NULL	0	NULL	1 equiv of electrophile	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With the vinyl boronates , the Zr-Csp2 bond is initially cleaved by 1 equiv of electrophile .
	manualset3
206094	1	417779	7	NULL	NULL	NULL	NULL	 model protein preparations	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	With these model protein preparations , the molar extinction coefficient of the ASB-protein complexes can be determined : the soluble ASB-RSA complexes can be brought to complete dissociation at pH 12.3 .
	manualset3
206095	2	417779	7	NULL	NULL	0	NULL	molar extinction coefficient 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With these model protein preparations , the molar extinction coefficient of the ASB-protein complexes can be determined : the soluble ASB-RSA complexes can be brought to complete dissociation at pH 12.3 .
	manualset3
206096	3	417779	7	NULL	NULL	0	NULL	ASB-protein complexes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	With these model protein preparations , the molar extinction coefficient of the ASB-protein complexes can be determined : the soluble ASB-RSA complexes can be brought to complete dissociation at pH 12.3 .
	manualset3
206097	4	417779	7	NULL	NULL	0	NULL	ASB-RSA complexes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	With these model protein preparations , the molar extinction coefficient of the ASB-protein complexes can be determined : the soluble ASB-RSA complexes can be brought to complete dissociation at pH 12.3 .
	manualset3
206098	5	417779	7	NULL	NULL	0	NULL	complete dissociation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With these model protein preparations , the molar extinction coefficient of the ASB-protein complexes can be determined : the soluble ASB-RSA complexes can be brought to complete dissociation at pH 12.3 .
	manualset3
206099	6	417779	7	NULL	NULL	0	NULL	 pH 12.3	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With these model protein preparations , the molar extinction coefficient of the ASB-protein complexes can be determined : the soluble ASB-RSA complexes can be brought to complete dissociation at pH 12.3 .
	manualset3
206100	1	417780	7	NULL	NULL	0	NULL	proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	With these proteins , the nucleotide excision repair enzyme XPG serves as a cofactor for the efficient function of hNth1 .
	manualset3
206101	2	417780	7	NULL	NULL	0	NULL	nucleotide excision repair enzyme XPG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	With these proteins , the nucleotide excision repair enzyme XPG serves as a cofactor for the efficient function of hNth1 .
	manualset3
206102	3	417780	7	NULL	NULL	0	NULL	cofactor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	With these proteins , the nucleotide excision repair enzyme XPG serves as a cofactor for the efficient function of hNth1 .
	manualset3
206103	4	417780	7	NULL	NULL	0	NULL	 efficient function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	With these proteins , the nucleotide excision repair enzyme XPG serves as a cofactor for the efficient function of hNth1 .
	manualset3
206104	5	417780	7	NULL	NULL	0	NULL	hNth1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	With these proteins , the nucleotide excision repair enzyme XPG serves as a cofactor for the efficient function of hNth1 .
	manualset3
206105	1	417781	7	NULL	NULL	0	NULL	approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	With this approach , only the inactive ( methylated ) PGK allele is selectively amplified by PCR .
	manualset3
206106	2	417781	7	NULL	NULL	0	NULL	 inactive ( methylated ) PGK allele	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	With this approach , only the inactive ( methylated ) PGK allele is selectively amplified by PCR .
	manualset3
206107	3	417781	7	NULL	NULL	0	NULL	PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	With this approach , only the inactive ( methylated ) PGK allele is selectively amplified by PCR .
	manualset3
206146	1	417782	7	NULL	NULL	0	NULL	long-term complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With this comes long-term complications of congenital heart disease such as the increased risk of atrial tachyarrhythmias .
	manualset3
206147	2	417782	7	NULL	NULL	0	NULL	congenital heart disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	With this comes long-term complications of congenital heart disease such as the increased risk of atrial tachyarrhythmias .
	manualset3
206149	3	417782	7	NULL	NULL	0	NULL	increased risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With this comes long-term complications of congenital heart disease such as the increased risk of atrial tachyarrhythmias .
	manualset3
206150	4	417782	7	NULL	NULL	0	NULL	atrial tachyarrhythmias	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With this comes long-term complications of congenital heart disease such as the increased risk of atrial tachyarrhythmias .
	manualset3
206151	1	417783	7	NULL	NULL	0	NULL	 fall	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With this fall in blood pressure there was a significant fall in activity of angiotensin-converting enzyme and in concentrations of plasma angiotensin II and aldosterone and a rise in plasma renin activity .
	manualset3
206152	2	417783	7	NULL	NULL	0	NULL	blood pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With this fall in blood pressure there was a significant fall in activity of angiotensin-converting enzyme and in concentrations of plasma angiotensin II and aldosterone and a rise in plasma renin activity .
	manualset3
206153	3	417783	7	NULL	NULL	0	NULL	 fall 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With this fall in blood pressure there was a significant fall in activity of angiotensin-converting enzyme and in concentrations of plasma angiotensin II and aldosterone and a rise in plasma renin activity .
	manualset3
206154	4	417783	7	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	With this fall in blood pressure there was a significant fall in activity of angiotensin-converting enzyme and in concentrations of plasma angiotensin II and aldosterone and a rise in plasma renin activity .
	manualset3
206155	5	417783	7	NULL	NULL	0	NULL	angiotensin-converting enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	With this fall in blood pressure there was a significant fall in activity of angiotensin-converting enzyme and in concentrations of plasma angiotensin II and aldosterone and a rise in plasma renin activity .
	manualset3
206156	6	417783	7	NULL	NULL	0	NULL	concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With this fall in blood pressure there was a significant fall in activity of angiotensin-converting enzyme and in concentrations of plasma angiotensin II and aldosterone and a rise in plasma renin activity .
	manualset3
206157	7	417783	7	NULL	NULL	0	NULL	plasma angiotensin II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	With this fall in blood pressure there was a significant fall in activity of angiotensin-converting enzyme and in concentrations of plasma angiotensin II and aldosterone and a rise in plasma renin activity .
	manualset3
206158	8	417783	7	NULL	NULL	0	NULL	aldosterone 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	With this fall in blood pressure there was a significant fall in activity of angiotensin-converting enzyme and in concentrations of plasma angiotensin II and aldosterone and a rise in plasma renin activity .
	manualset3
206159	9	417783	7	NULL	NULL	0	NULL	rise	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With this fall in blood pressure there was a significant fall in activity of angiotensin-converting enzyme and in concentrations of plasma angiotensin II and aldosterone and a rise in plasma renin activity .
	manualset3
206160	10	417783	7	NULL	NULL	0	NULL	plasma renin activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	With this fall in blood pressure there was a significant fall in activity of angiotensin-converting enzyme and in concentrations of plasma angiotensin II and aldosterone and a rise in plasma renin activity .
	manualset3
206161	1	417784	7	NULL	NULL	0	NULL	method	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	With this method , 16 obscure IUDs were removed , and 7 devices during pregnancy .
	manualset3
206162	2	417784	7	NULL	NULL	0	NULL	16 obscure IUDs	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	With this method , 16 obscure IUDs were removed , and 7 devices during pregnancy .
	manualset3
206163	3	417784	7	NULL	NULL	0	NULL	7 devices	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	With this method , 16 obscure IUDs were removed , and 7 devices during pregnancy .
	manualset3
206164	4	417784	7	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With this method , 16 obscure IUDs were removed , and 7 devices during pregnancy .
	manualset3
206165	1	417785	7	NULL	NULL	0	NULL	system 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	With this system we studied the instantaneous movement of the smoke cycle by cycle and that over a longer period .
	manualset3
206166	2	417785	7	NULL	NULL	0	NULL	 instantaneous movement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With this system we studied the instantaneous movement of the smoke cycle by cycle and that over a longer period .
	manualset3
206167	3	417785	7	NULL	NULL	NULL	NULL	smoke 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	With this system we studied the instantaneous movement of the smoke cycle by cycle and that over a longer period .
	manualset3
206168	4	417785	7	NULL	NULL	0	NULL	longer period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	With this system we studied the instantaneous movement of the smoke cycle by cycle and that over a longer period .
	manualset3
207907	5	417785	7	NULL	NULL	0	NULL	cycle by cycle	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With this system we studied the instantaneous movement of the smoke cycle by cycle and that over a longer period .
	manualset3
206169	1	417786	7	NULL	NULL	0	NULL	targeted DNA methylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	With this targeted DNA methylation and reporter system , we are able to monitor the progression of locus-specific DNA methylation in vivo and correlate such changes with potential functional changes .
	manualset3
206170	2	417786	7	NULL	NULL	0	NULL	reporter system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	With this targeted DNA methylation and reporter system , we are able to monitor the progression of locus-specific DNA methylation in vivo and correlate such changes with potential functional changes .
	manualset3
206171	3	417786	7	NULL	NULL	0	NULL	progression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	With this targeted DNA methylation and reporter system , we are able to monitor the progression of locus-specific DNA methylation in vivo and correlate such changes with potential functional changes .
	manualset3
206172	4	417786	7	NULL	NULL	0	NULL	locus-specific DNA methylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	With this targeted DNA methylation and reporter system , we are able to monitor the progression of locus-specific DNA methylation in vivo and correlate such changes with potential functional changes .
	manualset3
206173	5	417786	7	NULL	NULL	0	NULL	changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	With this targeted DNA methylation and reporter system , we are able to monitor the progression of locus-specific DNA methylation in vivo and correlate such changes with potential functional changes .
	manualset3
206174	6	417786	7	NULL	NULL	0	NULL	potential functional changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	With this targeted DNA methylation and reporter system , we are able to monitor the progression of locus-specific DNA methylation in vivo and correlate such changes with potential functional changes .
	manualset3
206175	1	417787	7	NULL	NULL	0	NULL	 therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	With this therapy the risk of hypoglycemia increased , but without inducing obvious clinical sequellae .
	manualset3
206176	2	417787	7	NULL	NULL	0	NULL	 risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With this therapy the risk of hypoglycemia increased , but without inducing obvious clinical sequellae .
	manualset3
206177	3	417787	7	NULL	NULL	0	NULL	hypoglycemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With this therapy the risk of hypoglycemia increased , but without inducing obvious clinical sequellae .
	manualset3
206178	4	417787	7	NULL	NULL	0	NULL	 clinical sequellae	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With this therapy the risk of hypoglycemia increased , but without inducing obvious clinical sequellae .
	manualset3
206179	1	417788	7	NULL	NULL	NULL	NULL	truncated receptor ,	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	With this truncated receptor , there is little if any additional GH-induced tyrosine phosphorylation of Jak2 or induced binding to the gamma response region .
	manualset3
206180	2	417788	7	NULL	NULL	0	NULL	GH-induced tyrosine phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	With this truncated receptor , there is little if any additional GH-induced tyrosine phosphorylation of Jak2 or induced binding to the gamma response region .
	manualset3
206181	3	417788	7	NULL	NULL	0	NULL	Jak2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	With this truncated receptor , there is little if any additional GH-induced tyrosine phosphorylation of Jak2 or induced binding to the gamma response region .
	manualset3
206182	4	417788	7	NULL	NULL	0	NULL	gamma response region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	With this truncated receptor , there is little if any additional GH-induced tyrosine phosphorylation of Jak2 or induced binding to the gamma response region .
	manualset3
207908	5	417788	7	NULL	NULL	0	NULL	induced binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	With this truncated receptor , there is little if any additional GH-induced tyrosine phosphorylation of Jak2 or induced binding to the gamma response region .
	manualset3
206183	1	417789	7	NULL	NULL	0	NULL	 veratryl alcohol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	With veratryl alcohol as an electron donor , the second-order rate constant for the formation of Compound II increased from 7.0.10 ( 3 ) M-1 .
	manualset3
206184	2	417789	7	NULL	NULL	0	NULL	electron donor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	With veratryl alcohol as an electron donor , the second-order rate constant for the formation of Compound II increased from 7.0.10 ( 3 ) M-1 .
	manualset3
206185	3	417789	7	NULL	NULL	0	NULL	second-order rate constant	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With veratryl alcohol as an electron donor , the second-order rate constant for the formation of Compound II increased from 7.0.10 ( 3 ) M-1 .
	manualset3
206186	4	417789	7	NULL	NULL	0	NULL	 formation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With veratryl alcohol as an electron donor , the second-order rate constant for the formation of Compound II increased from 7.0.10 ( 3 ) M-1 .
	manualset3
206187	5	417789	7	NULL	NULL	0	NULL	Compound II	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	With veratryl alcohol as an electron donor , the second-order rate constant for the formation of Compound II increased from 7.0.10 ( 3 ) M-1 .
	manualset3
206188	6	417789	7	NULL	NULL	0	NULL	7.0.10 ( 3 ) M-1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	With veratryl alcohol as an electron donor , the second-order rate constant for the formation of Compound II increased from 7.0.10 ( 3 ) M-1 .
	manualset3
206189	1	417790	7	NULL	NULL	0	NULL	Withdrawal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Withdrawal and withholding of medical treatment : Czech medical law at the crossroads .
	manualset3
206190	2	417790	7	NULL	NULL	0	NULL	withholding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Withdrawal and withholding of medical treatment : Czech medical law at the crossroads .
	manualset3
206191	3	417790	7	NULL	NULL	0	NULL	medical treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Withdrawal and withholding of medical treatment : Czech medical law at the crossroads .
	manualset3
206192	4	417790	7	NULL	NULL	0	NULL	Czech medical law	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Withdrawal and withholding of medical treatment : Czech medical law at the crossroads .
	manualset3
206193	5	417790	7	NULL	NULL	0	NULL	crossroads 	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Withdrawal and withholding of medical treatment : Czech medical law at the crossroads .
	manualset3
206194	1	417791	7	NULL	NULL	0	NULL	Withdrawal	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Withdrawal of blood-stained fluid , particularly if it contains tissue fragments , should alert the operator to the possibility of fetal damage .
	manualset3
206195	2	417791	7	NULL	NULL	0	NULL	blood-stained fluid	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Withdrawal of blood-stained fluid , particularly if it contains tissue fragments , should alert the operator to the possibility of fetal damage .
	manualset3
206196	3	417791	7	NULL	NULL	0	NULL	tissue fragments	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Withdrawal of blood-stained fluid , particularly if it contains tissue fragments , should alert the operator to the possibility of fetal damage .
	manualset3
206197	4	417791	7	NULL	NULL	0	NULL	operator	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Withdrawal of blood-stained fluid , particularly if it contains tissue fragments , should alert the operator to the possibility of fetal damage .
	manualset3
206198	5	417791	7	NULL	NULL	0	NULL	possibility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Withdrawal of blood-stained fluid , particularly if it contains tissue fragments , should alert the operator to the possibility of fetal damage .
	manualset3
206199	6	417791	7	NULL	NULL	0	NULL	fetal damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Withdrawal of blood-stained fluid , particularly if it contains tissue fragments , should alert the operator to the possibility of fetal damage .
	manualset3
206200	1	417792	7	NULL	NULL	0	NULL	24 h 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 24 h , alpha-GalCer induces a burst of IFN-gamma secretion in vivo , and recall with antigen in vitro leads to the synthesis of IL-4 and IL-10 in addition to IFN-gamma .
	manualset3
206201	2	417792	7	NULL	NULL	0	NULL	alpha-GalCer	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 24 h , alpha-GalCer induces a burst of IFN-gamma secretion in vivo , and recall with antigen in vitro leads to the synthesis of IL-4 and IL-10 in addition to IFN-gamma .
	manualset3
206202	3	417792	7	NULL	NULL	0	NULL	 IFN-gamma secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 24 h , alpha-GalCer induces a burst of IFN-gamma secretion in vivo , and recall with antigen in vitro leads to the synthesis of IL-4 and IL-10 in addition to IFN-gamma .
	manualset3
206203	4	417792	7	NULL	NULL	NULL	NULL	antigen	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Within 24 h , alpha-GalCer induces a burst of IFN-gamma secretion in vivo , and recall with antigen in vitro leads to the synthesis of IL-4 and IL-10 in addition to IFN-gamma .
	manualset3
206204	5	417792	7	NULL	NULL	0	NULL	synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 24 h , alpha-GalCer induces a burst of IFN-gamma secretion in vivo , and recall with antigen in vitro leads to the synthesis of IL-4 and IL-10 in addition to IFN-gamma .
	manualset3
206205	6	417792	7	NULL	NULL	0	NULL	IL-4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 24 h , alpha-GalCer induces a burst of IFN-gamma secretion in vivo , and recall with antigen in vitro leads to the synthesis of IL-4 and IL-10 in addition to IFN-gamma .
	manualset3
206206	7	417792	7	NULL	NULL	0	NULL	IL-10	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 24 h , alpha-GalCer induces a burst of IFN-gamma secretion in vivo , and recall with antigen in vitro leads to the synthesis of IL-4 and IL-10 in addition to IFN-gamma .
	manualset3
206207	8	417792	7	NULL	NULL	0	NULL	IFN-gamma	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 24 h , alpha-GalCer induces a burst of IFN-gamma secretion in vivo , and recall with antigen in vitro leads to the synthesis of IL-4 and IL-10 in addition to IFN-gamma .
	manualset3
207909	9	417792	7	NULL	NULL	NULL	NULL	burst	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Within 24 h , alpha-GalCer induces a burst of IFN-gamma secretion in vivo , and recall with antigen in vitro leads to the synthesis of IL-4 and IL-10 in addition to IFN-gamma .
	manualset3
206208	1	417793	7	NULL	NULL	0	NULL	24 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 24 h exogenous IGFBP-3 induced significant DNA fragmentation in RIN and HIT cells , at doses ranging from 4.4 to 2000 ng/ml ( P & lt ; 0.05 ) without a classic dose-response relationship .
	manualset3
206209	2	417793	7	NULL	NULL	0	NULL	exogenous IGFBP-3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 24 h exogenous IGFBP-3 induced significant DNA fragmentation in RIN and HIT cells , at doses ranging from 4.4 to 2000 ng/ml ( P & lt ; 0.05 ) without a classic dose-response relationship .
	manualset3
206210	3	417793	7	NULL	NULL	0	NULL	DNA fragmentation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 24 h exogenous IGFBP-3 induced significant DNA fragmentation in RIN and HIT cells , at doses ranging from 4.4 to 2000 ng/ml ( P & lt ; 0.05 ) without a classic dose-response relationship .
	manualset3
206211	4	417793	7	NULL	NULL	0	NULL	RIN cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 24 h exogenous IGFBP-3 induced significant DNA fragmentation in RIN and HIT cells , at doses ranging from 4.4 to 2000 ng/ml ( P & lt ; 0.05 ) without a classic dose-response relationship .
	manualset3
206212	5	417793	7	NULL	NULL	0	NULL	HIT cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 24 h exogenous IGFBP-3 induced significant DNA fragmentation in RIN and HIT cells , at doses ranging from 4.4 to 2000 ng/ml ( P & lt ; 0.05 ) without a classic dose-response relationship .
	manualset3
206213	6	417793	7	NULL	NULL	0	NULL	doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 24 h exogenous IGFBP-3 induced significant DNA fragmentation in RIN and HIT cells , at doses ranging from 4.4 to 2000 ng/ml ( P & lt ; 0.05 ) without a classic dose-response relationship .
	manualset3
206214	7	417793	7	NULL	NULL	0	NULL	4.4 ng/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 24 h exogenous IGFBP-3 induced significant DNA fragmentation in RIN and HIT cells , at doses ranging from 4.4 to 2000 ng/ml ( P & lt ; 0.05 ) without a classic dose-response relationship .
	manualset3
206215	8	417793	7	NULL	NULL	0	NULL	 2000 ng/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 24 h exogenous IGFBP-3 induced significant DNA fragmentation in RIN and HIT cells , at doses ranging from 4.4 to 2000 ng/ml ( P & lt ; 0.05 ) without a classic dose-response relationship .
	manualset3
206216	9	417793	7	NULL	NULL	0	NULL	P & lt ; 0.05	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 24 h exogenous IGFBP-3 induced significant DNA fragmentation in RIN and HIT cells , at doses ranging from 4.4 to 2000 ng/ml ( P & lt ; 0.05 ) without a classic dose-response relationship .
	manualset3
206217	10	417793	7	NULL	NULL	0	NULL	classic dose-response relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 24 h exogenous IGFBP-3 induced significant DNA fragmentation in RIN and HIT cells , at doses ranging from 4.4 to 2000 ng/ml ( P & lt ; 0.05 ) without a classic dose-response relationship .
	manualset3
206218	1	417794	7	NULL	NULL	0	NULL	24 h 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 24 h the patient developed fever , leucocytosis , impaired sense of smell and allodynia and hyperpathia in all 4 limbs .
	manualset3
206219	2	417794	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 24 h the patient developed fever , leucocytosis , impaired sense of smell and allodynia and hyperpathia in all 4 limbs .
	manualset3
206220	3	417794	7	NULL	NULL	0	NULL	fever	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 24 h the patient developed fever , leucocytosis , impaired sense of smell and allodynia and hyperpathia in all 4 limbs .
	manualset3
206221	4	417794	7	NULL	NULL	0	NULL	leucocytosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 24 h the patient developed fever , leucocytosis , impaired sense of smell and allodynia and hyperpathia in all 4 limbs .
	manualset3
206222	5	417794	7	NULL	NULL	0	NULL	impaired sense	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 24 h the patient developed fever , leucocytosis , impaired sense of smell and allodynia and hyperpathia in all 4 limbs .
	manualset3
206223	6	417794	7	NULL	NULL	0	NULL	smell	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 24 h the patient developed fever , leucocytosis , impaired sense of smell and allodynia and hyperpathia in all 4 limbs .
	manualset3
206224	7	417794	7	NULL	NULL	0	NULL	allodynia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 24 h the patient developed fever , leucocytosis , impaired sense of smell and allodynia and hyperpathia in all 4 limbs .
	manualset3
206225	8	417794	7	NULL	NULL	0	NULL	hyperpathia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 24 h the patient developed fever , leucocytosis , impaired sense of smell and allodynia and hyperpathia in all 4 limbs .
	manualset3
206226	9	417794	7	NULL	NULL	0	NULL	 4 limbs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 24 h the patient developed fever , leucocytosis , impaired sense of smell and allodynia and hyperpathia in all 4 limbs .
	manualset3
206227	1	417795	7	NULL	NULL	0	NULL	AML	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Within AML , French-American-British ( FAB ) M5 samples were most sensitive to tipifarnib .
	manualset3
206228	2	417795	7	NULL	NULL	0	NULL	French-American-British ( FAB ) M5 samples	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Within AML , French-American-British ( FAB ) M5 samples were most sensitive to tipifarnib .
	manualset3
206229	3	417795	7	NULL	NULL	0	NULL	tipifarnib	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Within AML , French-American-British ( FAB ) M5 samples were most sensitive to tipifarnib .
	manualset3
206230	1	417796	7	NULL	NULL	0	NULL	 group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Within each group , 10 rats were selected for treadmill running ( 60 % maximal O2 consumption , 1 h/day , 6 days/wk for 15 wk ) .
	manualset3
206231	2	417796	7	NULL	NULL	0	NULL	10 rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Within each group , 10 rats were selected for treadmill running ( 60 % maximal O2 consumption , 1 h/day , 6 days/wk for 15 wk ) .
	manualset3
206232	3	417796	7	NULL	NULL	0	NULL	treadmill running	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Within each group , 10 rats were selected for treadmill running ( 60 % maximal O2 consumption , 1 h/day , 6 days/wk for 15 wk ) .
	manualset3
206233	4	417796	7	NULL	NULL	0	NULL	60 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Within each group , 10 rats were selected for treadmill running ( 60 % maximal O2 consumption , 1 h/day , 6 days/wk for 15 wk ) .
	manualset3
206234	5	417796	7	NULL	NULL	0	NULL	maximal O2 consumption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Within each group , 10 rats were selected for treadmill running ( 60 % maximal O2 consumption , 1 h/day , 6 days/wk for 15 wk ) .
	manualset3
206235	6	417796	7	NULL	NULL	0	NULL	1 h/day	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Within each group , 10 rats were selected for treadmill running ( 60 % maximal O2 consumption , 1 h/day , 6 days/wk for 15 wk ) .
	manualset3
206236	7	417796	7	NULL	NULL	0	NULL	6 days/wk	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Within each group , 10 rats were selected for treadmill running ( 60 % maximal O2 consumption , 1 h/day , 6 days/wk for 15 wk ) .
	manualset3
206237	8	417796	7	NULL	NULL	0	NULL	15 wk	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Within each group , 10 rats were selected for treadmill running ( 60 % maximal O2 consumption , 1 h/day , 6 days/wk for 15 wk ) .
	manualset3
206238	1	417797	7	NULL	NULL	0	NULL	section	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Within each section , articles are listed in alphabetical order with respect to author ( 3 Weeks journals - Search completed at 28th .
	manualset3
206239	2	417797	7	NULL	NULL	0	NULL	articles	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Within each section , articles are listed in alphabetical order with respect to author ( 3 Weeks journals - Search completed at 28th .
	manualset3
206240	3	417797	7	NULL	NULL	0	NULL	alphabetical order	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Within each section , articles are listed in alphabetical order with respect to author ( 3 Weeks journals - Search completed at 28th .
	manualset3
206241	4	417797	7	NULL	NULL	0	NULL	author 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Within each section , articles are listed in alphabetical order with respect to author ( 3 Weeks journals - Search completed at 28th .
	manualset3
206242	5	417797	7	NULL	NULL	0	NULL	3 Weeks journals	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Within each section , articles are listed in alphabetical order with respect to author ( 3 Weeks journals - Search completed at 28th .
	manualset3
206243	6	417797	7	NULL	NULL	0	NULL	Search	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Within each section , articles are listed in alphabetical order with respect to author ( 3 Weeks journals - Search completed at 28th .
	manualset3
206244	7	417797	7	NULL	NULL	0	NULL	28th	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Within each section , articles are listed in alphabetical order with respect to author ( 3 Weeks journals - Search completed at 28th .
	manualset3
206245	1	417798	7	NULL	NULL	0	NULL	testing session	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Within each testing session , participants completed 3 trials of 1-leg standing with their dominant leg .
	manualset3
206246	2	417798	7	NULL	NULL	0	NULL	 participants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Within each testing session , participants completed 3 trials of 1-leg standing with their dominant leg .
	manualset3
206247	3	417798	7	NULL	NULL	0	NULL	3 trials 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Within each testing session , participants completed 3 trials of 1-leg standing with their dominant leg .
	manualset3
206248	4	417798	7	NULL	NULL	0	NULL	1-leg standing 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Within each testing session , participants completed 3 trials of 1-leg standing with their dominant leg .
	manualset3
206249	5	417798	7	NULL	NULL	0	NULL	dominant leg	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Within each testing session , participants completed 3 trials of 1-leg standing with their dominant leg .
	manualset3
206250	1	417799	7	NULL	NULL	0	NULL	specimens	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	All specimens showed a protruded nerve end .
	manualset3
206251	2	417799	7	NULL	NULL	0	NULL	protruded nerve end	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	All specimens showed a protruded nerve end .
	manualset3
206252	1	417800	7	NULL	NULL	0	NULL	minutes	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Within minutes of egg activation , dynamic actin-rich comet tails appeared on a subset of cytoplasmic vesicles that were enriched in protein kinase C ( PKC ) , causing the vesicles to move through the cytoplasm .
	manualset3
206253	2	417800	7	NULL	NULL	0	NULL	egg activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Within minutes of egg activation , dynamic actin-rich comet tails appeared on a subset of cytoplasmic vesicles that were enriched in protein kinase C ( PKC ) , causing the vesicles to move through the cytoplasm .
	manualset3
206254	3	417800	7	NULL	NULL	0	NULL	 dynamic actin-rich comet tails	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Within minutes of egg activation , dynamic actin-rich comet tails appeared on a subset of cytoplasmic vesicles that were enriched in protein kinase C ( PKC ) , causing the vesicles to move through the cytoplasm .
	manualset3
206255	4	417800	7	NULL	NULL	0	NULL	subset 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Within minutes of egg activation , dynamic actin-rich comet tails appeared on a subset of cytoplasmic vesicles that were enriched in protein kinase C ( PKC ) , causing the vesicles to move through the cytoplasm .
	manualset3
206256	5	417800	7	NULL	NULL	0	NULL	cytoplasmic vesicles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Within minutes of egg activation , dynamic actin-rich comet tails appeared on a subset of cytoplasmic vesicles that were enriched in protein kinase C ( PKC ) , causing the vesicles to move through the cytoplasm .
	manualset3
206257	6	417800	7	NULL	NULL	0	NULL	protein kinase C ( PKC )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Within minutes of egg activation , dynamic actin-rich comet tails appeared on a subset of cytoplasmic vesicles that were enriched in protein kinase C ( PKC ) , causing the vesicles to move through the cytoplasm .
	manualset3
206258	7	417800	7	NULL	NULL	0	NULL	 vesicles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Within minutes of egg activation , dynamic actin-rich comet tails appeared on a subset of cytoplasmic vesicles that were enriched in protein kinase C ( PKC ) , causing the vesicles to move through the cytoplasm .
	manualset3
206259	8	417800	7	NULL	NULL	0	NULL	cytoplasm	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Within minutes of egg activation , dynamic actin-rich comet tails appeared on a subset of cytoplasmic vesicles that were enriched in protein kinase C ( PKC ) , causing the vesicles to move through the cytoplasm .
	manualset3
206260	1	417801	7	NULL	NULL	0	NULL	nursing education 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Within nursing education , graduate pedagogies are relatively unexplored , with research commonly focused upon undergraduate and continuing education .
	manualset3
206261	2	417801	7	NULL	NULL	0	NULL	graduate pedagogies 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Within nursing education , graduate pedagogies are relatively unexplored , with research commonly focused upon undergraduate and continuing education .
	manualset3
206262	3	417801	7	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Within nursing education , graduate pedagogies are relatively unexplored , with research commonly focused upon undergraduate and continuing education .
	manualset3
206263	4	417801	7	NULL	NULL	0	NULL	undergraduate education	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Within nursing education , graduate pedagogies are relatively unexplored , with research commonly focused upon undergraduate and continuing education .
	manualset3
206264	5	417801	7	NULL	NULL	0	NULL	continuing education	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Within nursing education , graduate pedagogies are relatively unexplored , with research commonly focused upon undergraduate and continuing education .
	manualset3
206265	1	417802	7	NULL	NULL	0	NULL	enrichment context	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Within our enrichment context we find a phytosterol intake satiation , if multiple plant sterol-enriched foods are eaten .
	manualset3
206266	2	417802	7	NULL	NULL	0	NULL	phytosterol intake satiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Within our enrichment context we find a phytosterol intake satiation , if multiple plant sterol-enriched foods are eaten .
	manualset3
206267	3	417802	7	NULL	NULL	0	NULL	multiple plant sterol-enriched foods	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Within our enrichment context we find a phytosterol intake satiation , if multiple plant sterol-enriched foods are eaten .
	manualset3
206268	1	417803	7	NULL	NULL	NULL	NULL	segment I	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Within segment I the helix-turn-helix DNA-binding domain was mapped , whereas segment III was found to be nonessential .
	manualset3
206269	2	417803	7	NULL	NULL	0	NULL	helix-turn-helix DNA-binding domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Within segment I the helix-turn-helix DNA-binding domain was mapped , whereas segment III was found to be nonessential .
	manualset3
206270	3	417803	7	NULL	NULL	0	NULL	segment III	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Within segment I the helix-turn-helix DNA-binding domain was mapped , whereas segment III was found to be nonessential .
	manualset3
206271	1	417804	7	NULL	NULL	0	NULL	Rickettsia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the Rickettsia , ABM is confined to members of the spotted fever group ( SFG ) , such as Rickettsia rickettsii , the agent of Rocky Mountain spotted fever .
	manualset3
206272	2	417804	7	NULL	NULL	0	NULL	ABM	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the Rickettsia , ABM is confined to members of the spotted fever group ( SFG ) , such as Rickettsia rickettsii , the agent of Rocky Mountain spotted fever .
	manualset3
206273	3	417804	7	NULL	NULL	0	NULL	members	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the Rickettsia , ABM is confined to members of the spotted fever group ( SFG ) , such as Rickettsia rickettsii , the agent of Rocky Mountain spotted fever .
	manualset3
206274	4	417804	7	NULL	NULL	0	NULL	spotted fever group ( SFG )	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the Rickettsia , ABM is confined to members of the spotted fever group ( SFG ) , such as Rickettsia rickettsii , the agent of Rocky Mountain spotted fever .
	manualset3
206275	5	417804	7	NULL	NULL	0	NULL	Rickettsia rickettsii	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the Rickettsia , ABM is confined to members of the spotted fever group ( SFG ) , such as Rickettsia rickettsii , the agent of Rocky Mountain spotted fever .
	manualset3
206276	6	417804	7	NULL	NULL	0	NULL	 agent 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the Rickettsia , ABM is confined to members of the spotted fever group ( SFG ) , such as Rickettsia rickettsii , the agent of Rocky Mountain spotted fever .
	manualset3
206277	7	417804	7	NULL	NULL	0	NULL	Rocky Mountain spotted fever	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the Rickettsia , ABM is confined to members of the spotted fever group ( SFG ) , such as Rickettsia rickettsii , the agent of Rocky Mountain spotted fever .
	manualset3
206278	1	417805	7	NULL	NULL	0	NULL	aging population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the aging population , those with greatest health needs include members of minority groups , recent immigrants , and the old-old .
	manualset3
206279	2	417805	7	NULL	NULL	0	NULL	health needs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the aging population , those with greatest health needs include members of minority groups , recent immigrants , and the old-old .
	manualset3
206280	3	417805	7	NULL	NULL	0	NULL	members	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the aging population , those with greatest health needs include members of minority groups , recent immigrants , and the old-old .
	manualset3
206281	4	417805	7	NULL	NULL	0	NULL	minority groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the aging population , those with greatest health needs include members of minority groups , recent immigrants , and the old-old .
	manualset3
206282	5	417805	7	NULL	NULL	0	NULL	recent immigrants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the aging population , those with greatest health needs include members of minority groups , recent immigrants , and the old-old .
	manualset3
206283	6	417805	7	NULL	NULL	0	NULL	old-old	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the aging population , those with greatest health needs include members of minority groups , recent immigrants , and the old-old .
	manualset3
206390	1	417806	7	NULL	NULL	0	NULL	blunt trauma group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the blunt trauma group , eight of 18 injuries resulted in a competent airway and a good voice , six with a good airway but a fair voice , and four with airway compromise .
	manualset3
206391	2	417806	7	NULL	NULL	0	NULL	eight injuries	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the blunt trauma group , eight of 18 injuries resulted in a competent airway and a good voice , six with a good airway but a fair voice , and four with airway compromise .
	manualset3
206392	3	417806	7	NULL	NULL	0	NULL	18 injuries	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the blunt trauma group , eight of 18 injuries resulted in a competent airway and a good voice , six with a good airway but a fair voice , and four with airway compromise .
	manualset3
206393	4	417806	7	NULL	NULL	0	NULL	competent airway	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the blunt trauma group , eight of 18 injuries resulted in a competent airway and a good voice , six with a good airway but a fair voice , and four with airway compromise .
	manualset3
206394	5	417806	7	NULL	NULL	NULL	NULL	good voice	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Within the blunt trauma group , eight of 18 injuries resulted in a competent airway and a good voice , six with a good airway but a fair voice , and four with airway compromise .
	manualset3
206395	6	417806	7	NULL	NULL	0	NULL	six	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the blunt trauma group , eight of 18 injuries resulted in a competent airway and a good voice , six with a good airway but a fair voice , and four with airway compromise .
	manualset3
206396	7	417806	7	NULL	NULL	0	NULL	good airway 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the blunt trauma group , eight of 18 injuries resulted in a competent airway and a good voice , six with a good airway but a fair voice , and four with airway compromise .
	manualset3
206397	8	417806	7	NULL	NULL	0	NULL	fair voice	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the blunt trauma group , eight of 18 injuries resulted in a competent airway and a good voice , six with a good airway but a fair voice , and four with airway compromise .
	manualset3
206398	9	417806	7	NULL	NULL	0	NULL	four	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the blunt trauma group , eight of 18 injuries resulted in a competent airway and a good voice , six with a good airway but a fair voice , and four with airway compromise .
	manualset3
206399	10	417806	7	NULL	NULL	0	NULL	airway	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the blunt trauma group , eight of 18 injuries resulted in a competent airway and a good voice , six with a good airway but a fair voice , and four with airway compromise .
	manualset3
206400	1	417807	7	NULL	NULL	0	NULL	 context	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the context of this activity the SKLM also organises symposia and expert discussions , their outcome subsequently being published as resolutions , conclusions or opinions .
	manualset3
206401	2	417807	7	NULL	NULL	0	NULL	activity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the context of this activity the SKLM also organises symposia and expert discussions , their outcome subsequently being published as resolutions , conclusions or opinions .
	manualset3
206402	3	417807	7	NULL	NULL	0	NULL	SKLM	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the context of this activity the SKLM also organises symposia and expert discussions , their outcome subsequently being published as resolutions , conclusions or opinions .
	manualset3
206403	4	417807	7	NULL	NULL	0	NULL	symposia	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the context of this activity the SKLM also organises symposia and expert discussions , their outcome subsequently being published as resolutions , conclusions or opinions .
	manualset3
206404	5	417807	7	NULL	NULL	0	NULL	expert discussions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the context of this activity the SKLM also organises symposia and expert discussions , their outcome subsequently being published as resolutions , conclusions or opinions .
	manualset3
206405	6	417807	7	NULL	NULL	0	NULL	outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the context of this activity the SKLM also organises symposia and expert discussions , their outcome subsequently being published as resolutions , conclusions or opinions .
	manualset3
206406	7	417807	7	NULL	NULL	0	NULL	 resolutions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the context of this activity the SKLM also organises symposia and expert discussions , their outcome subsequently being published as resolutions , conclusions or opinions .
	manualset3
206407	8	417807	7	NULL	NULL	0	NULL	conclusions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the context of this activity the SKLM also organises symposia and expert discussions , their outcome subsequently being published as resolutions , conclusions or opinions .
	manualset3
206408	9	417807	7	NULL	NULL	0	NULL	 opinions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the context of this activity the SKLM also organises symposia and expert discussions , their outcome subsequently being published as resolutions , conclusions or opinions .
	manualset3
206409	1	417808	7	NULL	NULL	0	NULL	 detector	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the detector , cone signals are distinguished from rod-related activity and intrinsic dark noise on the basis of signal-to-noise discriminations .5 .
	manualset3
206410	2	417808	7	NULL	NULL	0	NULL	cone signals	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the detector , cone signals are distinguished from rod-related activity and intrinsic dark noise on the basis of signal-to-noise discriminations .5 .
	manualset3
206411	3	417808	7	NULL	NULL	NULL	NULL	rod-related activity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Within the detector , cone signals are distinguished from rod-related activity and intrinsic dark noise on the basis of signal-to-noise discriminations .5 .
	manualset3
206412	4	417808	7	NULL	NULL	0	NULL	 intrinsic dark noise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the detector , cone signals are distinguished from rod-related activity and intrinsic dark noise on the basis of signal-to-noise discriminations .5 .
	manualset3
206413	5	417808	7	NULL	NULL	0	NULL	 basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the detector , cone signals are distinguished from rod-related activity and intrinsic dark noise on the basis of signal-to-noise discriminations .5 .
	manualset3
206414	6	417808	7	NULL	NULL	0	NULL	signal-to-noise discriminations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the detector , cone signals are distinguished from rod-related activity and intrinsic dark noise on the basis of signal-to-noise discriminations .5 .
	manualset3
206415	7	417808	7	NULL	NULL	0	NULL	.5	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the detector , cone signals are distinguished from rod-related activity and intrinsic dark noise on the basis of signal-to-noise discriminations .5 .
	manualset3
206416	1	417809	7	NULL	NULL	0	NULL	 recurrent model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the recurrent model , stimulus detection was characterized by a relatively early strength increase of the feedforward connection from primary to secondary somatosensory cortex ( & gt ; 80 ms ) .
	manualset3
206417	2	417809	7	NULL	NULL	0	NULL	stimulus detection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the recurrent model , stimulus detection was characterized by a relatively early strength increase of the feedforward connection from primary to secondary somatosensory cortex ( & gt ; 80 ms ) .
	manualset3
206418	3	417809	7	NULL	NULL	0	NULL	early strength increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the recurrent model , stimulus detection was characterized by a relatively early strength increase of the feedforward connection from primary to secondary somatosensory cortex ( & gt ; 80 ms ) .
	manualset3
206419	4	417809	7	NULL	NULL	0	NULL	feedforward connection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the recurrent model , stimulus detection was characterized by a relatively early strength increase of the feedforward connection from primary to secondary somatosensory cortex ( & gt ; 80 ms ) .
	manualset3
206420	5	417809	7	NULL	NULL	0	NULL	primary cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the recurrent model , stimulus detection was characterized by a relatively early strength increase of the feedforward connection from primary to secondary somatosensory cortex ( & gt ; 80 ms ) .
	manualset3
206421	6	417809	7	NULL	NULL	0	NULL	secondary somatosensory cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the recurrent model , stimulus detection was characterized by a relatively early strength increase of the feedforward connection from primary to secondary somatosensory cortex ( & gt ; 80 ms ) .
	manualset3
206422	7	417809	7	NULL	NULL	0	NULL	& gt ; 80 ms	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the recurrent model , stimulus detection was characterized by a relatively early strength increase of the feedforward connection from primary to secondary somatosensory cortex ( & gt ; 80 ms ) .
	manualset3
206423	1	417810	7	NULL	NULL	0	NULL	strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the strains tested , viruses of subtypes I-ABC and I-D were lethal for guinea pigs , and viruses of other subtypes were benign .
	manualset3
206424	2	417810	7	NULL	NULL	0	NULL	viruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the strains tested , viruses of subtypes I-ABC and I-D were lethal for guinea pigs , and viruses of other subtypes were benign .
	manualset3
206425	3	417810	7	NULL	NULL	0	NULL	subtypes I-ABC	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the strains tested , viruses of subtypes I-ABC and I-D were lethal for guinea pigs , and viruses of other subtypes were benign .
	manualset3
206426	4	417810	7	NULL	NULL	0	NULL	I-D	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the strains tested , viruses of subtypes I-ABC and I-D were lethal for guinea pigs , and viruses of other subtypes were benign .
	manualset3
206427	5	417810	7	NULL	NULL	0	NULL	guinea pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the strains tested , viruses of subtypes I-ABC and I-D were lethal for guinea pigs , and viruses of other subtypes were benign .
	manualset3
206428	6	417810	7	NULL	NULL	0	NULL	 viruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the strains tested , viruses of subtypes I-ABC and I-D were lethal for guinea pigs , and viruses of other subtypes were benign .
	manualset3
206429	7	417810	7	NULL	NULL	0	NULL	subtypes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the strains tested , viruses of subtypes I-ABC and I-D were lethal for guinea pigs , and viruses of other subtypes were benign .
	manualset3
206430	1	417811	7	NULL	NULL	0	NULL	group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Within this group , 65 protein signals showed significant changes compared to controls already at 1 % lethal concentration ( LC ( 01 ) ) .
	manualset3
206431	2	417811	7	NULL	NULL	0	NULL	65 protein signals	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Within this group , 65 protein signals showed significant changes compared to controls already at 1 % lethal concentration ( LC ( 01 ) ) .
	manualset3
206432	3	417811	7	NULL	NULL	0	NULL	controls 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Within this group , 65 protein signals showed significant changes compared to controls already at 1 % lethal concentration ( LC ( 01 ) ) .
	manualset3
206433	4	417811	7	NULL	NULL	0	NULL	1 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Within this group , 65 protein signals showed significant changes compared to controls already at 1 % lethal concentration ( LC ( 01 ) ) .
	manualset3
206434	5	417811	7	NULL	NULL	0	NULL	lethal concentration ( LC ( 01 ) )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Within this group , 65 protein signals showed significant changes compared to controls already at 1 % lethal concentration ( LC ( 01 ) ) .
	manualset3
206435	1	417812	7	NULL	NULL	0	NULL	precautions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Without precautions especially , the oxalate concentration in urine may be doubled or tripled during one day of storage .
	manualset3
206436	2	417812	7	NULL	NULL	0	NULL	oxalate concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Without precautions especially , the oxalate concentration in urine may be doubled or tripled during one day of storage .
	manualset3
206437	3	417812	7	NULL	NULL	0	NULL	 urine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Without precautions especially , the oxalate concentration in urine may be doubled or tripled during one day of storage .
	manualset3
206438	4	417812	7	NULL	NULL	0	NULL	one day	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Without precautions especially , the oxalate concentration in urine may be doubled or tripled during one day of storage .
	manualset3
206439	5	417812	7	NULL	NULL	0	NULL	storage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Without precautions especially , the oxalate concentration in urine may be doubled or tripled during one day of storage .
	manualset3
206440	1	417813	7	NULL	NULL	0	NULL	 stones 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All stones in the upper third of the ureter and larger stones in the distal third of the ureter are preferably treated with ESWL in situ whereas smaller stones in the distal ureter are better treated endoscopically .
	manualset3
206441	2	417813	7	NULL	NULL	0	NULL	upper third 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	All stones in the upper third of the ureter and larger stones in the distal third of the ureter are preferably treated with ESWL in situ whereas smaller stones in the distal ureter are better treated endoscopically .
	manualset3
206442	3	417813	7	NULL	NULL	0	NULL	ureter 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	All stones in the upper third of the ureter and larger stones in the distal third of the ureter are preferably treated with ESWL in situ whereas smaller stones in the distal ureter are better treated endoscopically .
	manualset3
206443	4	417813	7	NULL	NULL	0	NULL	larger stones	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All stones in the upper third of the ureter and larger stones in the distal third of the ureter are preferably treated with ESWL in situ whereas smaller stones in the distal ureter are better treated endoscopically .
	manualset3
206444	5	417813	7	NULL	NULL	0	NULL	distal third	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	All stones in the upper third of the ureter and larger stones in the distal third of the ureter are preferably treated with ESWL in situ whereas smaller stones in the distal ureter are better treated endoscopically .
	manualset3
206445	6	417813	7	NULL	NULL	0	NULL	 ureter	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	All stones in the upper third of the ureter and larger stones in the distal third of the ureter are preferably treated with ESWL in situ whereas smaller stones in the distal ureter are better treated endoscopically .
	manualset3
206446	7	417813	7	NULL	NULL	0	NULL	ESWL	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All stones in the upper third of the ureter and larger stones in the distal third of the ureter are preferably treated with ESWL in situ whereas smaller stones in the distal ureter are better treated endoscopically .
	manualset3
206447	8	417813	7	NULL	NULL	0	NULL	smaller stones	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All stones in the upper third of the ureter and larger stones in the distal third of the ureter are preferably treated with ESWL in situ whereas smaller stones in the distal ureter are better treated endoscopically .
	manualset3
206448	9	417813	7	NULL	NULL	0	NULL	distal ureter	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	All stones in the upper third of the ureter and larger stones in the distal third of the ureter are preferably treated with ESWL in situ whereas smaller stones in the distal ureter are better treated endoscopically .
	manualset3
206449	1	417814	7	NULL	NULL	0	NULL	Wizardry beliefs	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Wizardry beliefs are seen by Mutumwa Nchimi healers to reflect the problems faced by urban dwellers in particular who , on the one hand , find themselves afflicted by feelings of shame or guilt with respect to failure to observe traditional morality and , on the other hand , by an awareness of suspected rival forces in the competitive urban environment .
	manualset3
206450	2	417814	7	NULL	NULL	0	NULL	Mutumwa Nchimi healers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Wizardry beliefs are seen by Mutumwa Nchimi healers to reflect the problems faced by urban dwellers in particular who , on the one hand , find themselves afflicted by feelings of shame or guilt with respect to failure to observe traditional morality and , on the other hand , by an awareness of suspected rival forces in the competitive urban environment .
	manualset3
206451	3	417814	7	NULL	NULL	0	NULL	problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Wizardry beliefs are seen by Mutumwa Nchimi healers to reflect the problems faced by urban dwellers in particular who , on the one hand , find themselves afflicted by feelings of shame or guilt with respect to failure to observe traditional morality and , on the other hand , by an awareness of suspected rival forces in the competitive urban environment .
	manualset3
206452	4	417814	7	NULL	NULL	0	NULL	urban dwellers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Wizardry beliefs are seen by Mutumwa Nchimi healers to reflect the problems faced by urban dwellers in particular who , on the one hand , find themselves afflicted by feelings of shame or guilt with respect to failure to observe traditional morality and , on the other hand , by an awareness of suspected rival forces in the competitive urban environment .
	manualset3
206454	6	417814	7	NULL	NULL	0	NULL	feelings of shame	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Wizardry beliefs are seen by Mutumwa Nchimi healers to reflect the problems faced by urban dwellers in particular who , on the one hand , find themselves afflicted by feelings of shame or guilt with respect to failure to observe traditional morality and , on the other hand , by an awareness of suspected rival forces in the competitive urban environment .
	manualset3
206455	7	417814	7	NULL	NULL	0	NULL	feelings of guilt	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Wizardry beliefs are seen by Mutumwa Nchimi healers to reflect the problems faced by urban dwellers in particular who , on the one hand , find themselves afflicted by feelings of shame or guilt with respect to failure to observe traditional morality and , on the other hand , by an awareness of suspected rival forces in the competitive urban environment .
	manualset3
206456	8	417814	7	NULL	NULL	0	NULL	failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Wizardry beliefs are seen by Mutumwa Nchimi healers to reflect the problems faced by urban dwellers in particular who , on the one hand , find themselves afflicted by feelings of shame or guilt with respect to failure to observe traditional morality and , on the other hand , by an awareness of suspected rival forces in the competitive urban environment .
	manualset3
206457	9	417814	7	NULL	NULL	0	NULL	traditional morality	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Wizardry beliefs are seen by Mutumwa Nchimi healers to reflect the problems faced by urban dwellers in particular who , on the one hand , find themselves afflicted by feelings of shame or guilt with respect to failure to observe traditional morality and , on the other hand , by an awareness of suspected rival forces in the competitive urban environment .
	manualset3
206459	11	417814	7	NULL	NULL	NULL	NULL	awareness	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Wizardry beliefs are seen by Mutumwa Nchimi healers to reflect the problems faced by urban dwellers in particular who , on the one hand , find themselves afflicted by feelings of shame or guilt with respect to failure to observe traditional morality and , on the other hand , by an awareness of suspected rival forces in the competitive urban environment .
	manualset3
206460	12	417814	7	NULL	NULL	0	NULL	suspected rival forces	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Wizardry beliefs are seen by Mutumwa Nchimi healers to reflect the problems faced by urban dwellers in particular who , on the one hand , find themselves afflicted by feelings of shame or guilt with respect to failure to observe traditional morality and , on the other hand , by an awareness of suspected rival forces in the competitive urban environment .
	manualset3
206462	13	417814	7	NULL	NULL	0	NULL	competitive urban environment 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Wizardry beliefs are seen by Mutumwa Nchimi healers to reflect the problems faced by urban dwellers in particular who , on the one hand , find themselves afflicted by feelings of shame or guilt with respect to failure to observe traditional morality and , on the other hand , by an awareness of suspected rival forces in the competitive urban environment .
	manualset3
206575	1	417815	7	NULL	NULL	0	NULL	Women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Women and the obstructive sleep apnea syndrome .
	manualset3
206576	2	417815	7	NULL	NULL	0	NULL	obstructive sleep apnea syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Women and the obstructive sleep apnea syndrome .
	manualset3
206577	1	417816	7	NULL	NULL	0	NULL	Women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Women attending 2 family planning clinics in Nairobi , Kenya , were enrolled in a study of risk factors for HIV infection between October 1989 and May 1991 .
	manualset3
206578	2	417816	7	NULL	NULL	0	NULL	2 family planning clinics	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Women attending 2 family planning clinics in Nairobi , Kenya , were enrolled in a study of risk factors for HIV infection between October 1989 and May 1991 .
	manualset3
206579	3	417816	7	NULL	NULL	0	NULL	Nairobi , Kenya 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Women attending 2 family planning clinics in Nairobi , Kenya , were enrolled in a study of risk factors for HIV infection between October 1989 and May 1991 .
	manualset3
206580	4	417816	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Women attending 2 family planning clinics in Nairobi , Kenya , were enrolled in a study of risk factors for HIV infection between October 1989 and May 1991 .
	manualset3
206581	5	417816	7	NULL	NULL	0	NULL	risk factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Women attending 2 family planning clinics in Nairobi , Kenya , were enrolled in a study of risk factors for HIV infection between October 1989 and May 1991 .
	manualset3
206582	6	417816	7	NULL	NULL	0	NULL	HIV infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Women attending 2 family planning clinics in Nairobi , Kenya , were enrolled in a study of risk factors for HIV infection between October 1989 and May 1991 .
	manualset3
206583	7	417816	7	NULL	NULL	0	NULL	October 1989	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Women attending 2 family planning clinics in Nairobi , Kenya , were enrolled in a study of risk factors for HIV infection between October 1989 and May 1991 .
	manualset3
206584	8	417816	7	NULL	NULL	0	NULL	May 1991	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Women attending 2 family planning clinics in Nairobi , Kenya , were enrolled in a study of risk factors for HIV infection between October 1989 and May 1991 .
	manualset3
206585	1	417817	7	NULL	NULL	0	NULL	Women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Women bear the burden of a family 's daily life , are more vulnerable than men , and face additional problems in the work force .
	manualset3
206586	2	417817	7	NULL	NULL	0	NULL	 burden	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Women bear the burden of a family 's daily life , are more vulnerable than men , and face additional problems in the work force .
	manualset3
206587	3	417817	7	NULL	NULL	0	NULL	family 's daily life	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Women bear the burden of a family 's daily life , are more vulnerable than men , and face additional problems in the work force .
	manualset3
206588	4	417817	7	NULL	NULL	0	NULL	 men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Women bear the burden of a family 's daily life , are more vulnerable than men , and face additional problems in the work force .
	manualset3
206589	5	417817	7	NULL	NULL	0	NULL	problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Women bear the burden of a family 's daily life , are more vulnerable than men , and face additional problems in the work force .
	manualset3
206590	6	417817	7	NULL	NULL	NULL	NULL	work force	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Women bear the burden of a family 's daily life , are more vulnerable than men , and face additional problems in the work force .
	manualset3
206591	1	417818	7	NULL	NULL	0	NULL	Women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Women must participate collectively and help develop and implement prevention strategies designed to increase their degree of empowerment and reduce their risk of exposure to HIV and AIDS .
	manualset3
206592	2	417818	7	NULL	NULL	0	NULL	prevention strategies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Women must participate collectively and help develop and implement prevention strategies designed to increase their degree of empowerment and reduce their risk of exposure to HIV and AIDS .
	manualset3
206593	3	417818	7	NULL	NULL	0	NULL	degree 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Women must participate collectively and help develop and implement prevention strategies designed to increase their degree of empowerment and reduce their risk of exposure to HIV and AIDS .
	manualset3
206594	4	417818	7	NULL	NULL	0	NULL	empowerment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Women must participate collectively and help develop and implement prevention strategies designed to increase their degree of empowerment and reduce their risk of exposure to HIV and AIDS .
	manualset3
206595	5	417818	7	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Women must participate collectively and help develop and implement prevention strategies designed to increase their degree of empowerment and reduce their risk of exposure to HIV and AIDS .
	manualset3
206596	6	417818	7	NULL	NULL	0	NULL	 exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Women must participate collectively and help develop and implement prevention strategies designed to increase their degree of empowerment and reduce their risk of exposure to HIV and AIDS .
	manualset3
206597	7	417818	7	NULL	NULL	0	NULL	HIV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Women must participate collectively and help develop and implement prevention strategies designed to increase their degree of empowerment and reduce their risk of exposure to HIV and AIDS .
	manualset3
206598	8	417818	7	NULL	NULL	0	NULL	AIDS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Women must participate collectively and help develop and implement prevention strategies designed to increase their degree of empowerment and reduce their risk of exposure to HIV and AIDS .
	manualset3
206599	1	417819	7	NULL	NULL	0	NULL	subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All subjects completed tests to assess verbal memory , attention , and executive functions .
	manualset3
206600	2	417819	7	NULL	NULL	0	NULL	 tests 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All subjects completed tests to assess verbal memory , attention , and executive functions .
	manualset3
206601	3	417819	7	NULL	NULL	0	NULL	verbal memory	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All subjects completed tests to assess verbal memory , attention , and executive functions .
	manualset3
206602	4	417819	7	NULL	NULL	0	NULL	attention	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All subjects completed tests to assess verbal memory , attention , and executive functions .
	manualset3
206603	5	417819	7	NULL	NULL	0	NULL	executive functions	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All subjects completed tests to assess verbal memory , attention , and executive functions .
	manualset3
206604	1	417820	7	NULL	NULL	0	NULL	Women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Women reported more pain than men .
	manualset3
206605	2	417820	7	NULL	NULL	0	NULL	pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Women reported more pain than men .
	manualset3
206606	3	417820	7	NULL	NULL	0	NULL	 men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Women reported more pain than men .
	manualset3
206607	1	417821	7	NULL	NULL	0	NULL	Women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Women using nerve medicine and reporting depression twice had an odds ratio of 4.4 ( 95 % CI 1.1-17 .7 ) for sustaining a non-vertebral fracture , and those using nerve medicine and reporting coping problems twice had a corresponding OR 4.7 ( 95 % CI 1.2-18 .4 ) .
	manualset3
206608	2	417821	7	NULL	NULL	0	NULL	nerve medicine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Women using nerve medicine and reporting depression twice had an odds ratio of 4.4 ( 95 % CI 1.1-17 .7 ) for sustaining a non-vertebral fracture , and those using nerve medicine and reporting coping problems twice had a corresponding OR 4.7 ( 95 % CI 1.2-18 .4 ) .
	manualset3
206609	3	417821	7	NULL	NULL	0	NULL	depression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Women using nerve medicine and reporting depression twice had an odds ratio of 4.4 ( 95 % CI 1.1-17 .7 ) for sustaining a non-vertebral fracture , and those using nerve medicine and reporting coping problems twice had a corresponding OR 4.7 ( 95 % CI 1.2-18 .4 ) .
	manualset3
206610	4	417821	7	NULL	NULL	0	NULL	odds ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Women using nerve medicine and reporting depression twice had an odds ratio of 4.4 ( 95 % CI 1.1-17 .7 ) for sustaining a non-vertebral fracture , and those using nerve medicine and reporting coping problems twice had a corresponding OR 4.7 ( 95 % CI 1.2-18 .4 ) .
	manualset3
206611	5	417821	7	NULL	NULL	0	NULL	4.4 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Women using nerve medicine and reporting depression twice had an odds ratio of 4.4 ( 95 % CI 1.1-17 .7 ) for sustaining a non-vertebral fracture , and those using nerve medicine and reporting coping problems twice had a corresponding OR 4.7 ( 95 % CI 1.2-18 .4 ) .
	manualset3
206612	6	417821	7	NULL	NULL	0	NULL	95 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Women using nerve medicine and reporting depression twice had an odds ratio of 4.4 ( 95 % CI 1.1-17 .7 ) for sustaining a non-vertebral fracture , and those using nerve medicine and reporting coping problems twice had a corresponding OR 4.7 ( 95 % CI 1.2-18 .4 ) .
	manualset3
206613	7	417821	7	NULL	NULL	0	NULL	CI 1.1-17 .7	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Women using nerve medicine and reporting depression twice had an odds ratio of 4.4 ( 95 % CI 1.1-17 .7 ) for sustaining a non-vertebral fracture , and those using nerve medicine and reporting coping problems twice had a corresponding OR 4.7 ( 95 % CI 1.2-18 .4 ) .
	manualset3
206614	8	417821	7	NULL	NULL	0	NULL	non-vertebral fracture	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Women using nerve medicine and reporting depression twice had an odds ratio of 4.4 ( 95 % CI 1.1-17 .7 ) for sustaining a non-vertebral fracture , and those using nerve medicine and reporting coping problems twice had a corresponding OR 4.7 ( 95 % CI 1.2-18 .4 ) .
	manualset3
206615	9	417821	7	NULL	NULL	0	NULL	nerve medicine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Women using nerve medicine and reporting depression twice had an odds ratio of 4.4 ( 95 % CI 1.1-17 .7 ) for sustaining a non-vertebral fracture , and those using nerve medicine and reporting coping problems twice had a corresponding OR 4.7 ( 95 % CI 1.2-18 .4 ) .
	manualset3
206616	10	417821	7	NULL	NULL	0	NULL	coping problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Women using nerve medicine and reporting depression twice had an odds ratio of 4.4 ( 95 % CI 1.1-17 .7 ) for sustaining a non-vertebral fracture , and those using nerve medicine and reporting coping problems twice had a corresponding OR 4.7 ( 95 % CI 1.2-18 .4 ) .
	manualset3
206617	11	417821	7	NULL	NULL	NULL	NULL	 4.7	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Women using nerve medicine and reporting depression twice had an odds ratio of 4.4 ( 95 % CI 1.1-17 .7 ) for sustaining a non-vertebral fracture , and those using nerve medicine and reporting coping problems twice had a corresponding OR 4.7 ( 95 % CI 1.2-18 .4 ) .
	manualset3
206618	12	417821	7	NULL	NULL	0	NULL	95 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Women using nerve medicine and reporting depression twice had an odds ratio of 4.4 ( 95 % CI 1.1-17 .7 ) for sustaining a non-vertebral fracture , and those using nerve medicine and reporting coping problems twice had a corresponding OR 4.7 ( 95 % CI 1.2-18 .4 ) .
	manualset3
206619	13	417821	7	NULL	NULL	0	NULL	CI 1.2-18 .4 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Women using nerve medicine and reporting depression twice had an odds ratio of 4.4 ( 95 % CI 1.1-17 .7 ) for sustaining a non-vertebral fracture , and those using nerve medicine and reporting coping problems twice had a corresponding OR 4.7 ( 95 % CI 1.2-18 .4 ) .
	manualset3
206620	14	417821	7	NULL	NULL	0	NULL	OR	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Women using nerve medicine and reporting depression twice had an odds ratio of 4.4 ( 95 % CI 1.1-17 .7 ) for sustaining a non-vertebral fracture , and those using nerve medicine and reporting coping problems twice had a corresponding OR 4.7 ( 95 % CI 1.2-18 .4 ) .
	manualset3
206621	1	417822	7	NULL	NULL	0	NULL	Women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Women were weighed at 6 weeks , 3 months , and every 3 months thereafter for up to 24 months postpartum and data on mortality up to 2 years were collected .
	manualset3
206622	2	417822	7	NULL	NULL	0	NULL	6 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Women were weighed at 6 weeks , 3 months , and every 3 months thereafter for up to 24 months postpartum and data on mortality up to 2 years were collected .
	manualset3
206623	3	417822	7	NULL	NULL	0	NULL	3 months 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Women were weighed at 6 weeks , 3 months , and every 3 months thereafter for up to 24 months postpartum and data on mortality up to 2 years were collected .
	manualset3
206624	4	417822	7	NULL	NULL	0	NULL	3 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Women were weighed at 6 weeks , 3 months , and every 3 months thereafter for up to 24 months postpartum and data on mortality up to 2 years were collected .
	manualset3
206625	5	417822	7	NULL	NULL	0	NULL	 24 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Women were weighed at 6 weeks , 3 months , and every 3 months thereafter for up to 24 months postpartum and data on mortality up to 2 years were collected .
	manualset3
206626	6	417822	7	NULL	NULL	0	NULL	postpartum	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Women were weighed at 6 weeks , 3 months , and every 3 months thereafter for up to 24 months postpartum and data on mortality up to 2 years were collected .
	manualset3
206627	7	417822	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Women were weighed at 6 weeks , 3 months , and every 3 months thereafter for up to 24 months postpartum and data on mortality up to 2 years were collected .
	manualset3
206628	8	417822	7	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Women were weighed at 6 weeks , 3 months , and every 3 months thereafter for up to 24 months postpartum and data on mortality up to 2 years were collected .
	manualset3
206629	9	417822	7	NULL	NULL	0	NULL	2 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Women were weighed at 6 weeks , 3 months , and every 3 months thereafter for up to 24 months postpartum and data on mortality up to 2 years were collected .
	manualset3
206630	1	417823	7	NULL	NULL	0	NULL	Women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Women who stop smoking greatly reduce their risk of heart disease and other smoking-related illnesses .
	manualset3
206631	2	417823	7	NULL	NULL	0	NULL	smoking	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Women who stop smoking greatly reduce their risk of heart disease and other smoking-related illnesses .
	manualset3
206632	3	417823	7	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Women who stop smoking greatly reduce their risk of heart disease and other smoking-related illnesses .
	manualset3
206633	4	417823	7	NULL	NULL	0	NULL	heart disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Women who stop smoking greatly reduce their risk of heart disease and other smoking-related illnesses .
	manualset3
206634	5	417823	7	NULL	NULL	0	NULL	smoking-related illnesses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Women who stop smoking greatly reduce their risk of heart disease and other smoking-related illnesses .
	manualset3
206715	1	417824	7	NULL	NULL	0	NULL	Women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Women with operable early-stage breast cancer were enrolled in a multicenter study of neoadjuvant therapy for four 21-day cycles with capecitabine 825mg/m ( 2 ) plus docetaxel 75mg/m ( 2 ) if human epidermal growth factor receptor 2 ( HER2 ) - negative , and additionally , a standard trastuzumab dose if HER2-positive .
	manualset3
206716	2	417824	7	NULL	NULL	0	NULL	operable early-stage breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Women with operable early-stage breast cancer were enrolled in a multicenter study of neoadjuvant therapy for four 21-day cycles with capecitabine 825mg/m ( 2 ) plus docetaxel 75mg/m ( 2 ) if human epidermal growth factor receptor 2 ( HER2 ) - negative , and additionally , a standard trastuzumab dose if HER2-positive .
	manualset3
206717	3	417824	7	NULL	NULL	0	NULL	multicenter study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Women with operable early-stage breast cancer were enrolled in a multicenter study of neoadjuvant therapy for four 21-day cycles with capecitabine 825mg/m ( 2 ) plus docetaxel 75mg/m ( 2 ) if human epidermal growth factor receptor 2 ( HER2 ) - negative , and additionally , a standard trastuzumab dose if HER2-positive .
	manualset3
206718	4	417824	7	NULL	NULL	0	NULL	neoadjuvant therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Women with operable early-stage breast cancer were enrolled in a multicenter study of neoadjuvant therapy for four 21-day cycles with capecitabine 825mg/m ( 2 ) plus docetaxel 75mg/m ( 2 ) if human epidermal growth factor receptor 2 ( HER2 ) - negative , and additionally , a standard trastuzumab dose if HER2-positive .
	manualset3
206719	5	417824	7	NULL	NULL	0	NULL	four 21-day cycles	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Women with operable early-stage breast cancer were enrolled in a multicenter study of neoadjuvant therapy for four 21-day cycles with capecitabine 825mg/m ( 2 ) plus docetaxel 75mg/m ( 2 ) if human epidermal growth factor receptor 2 ( HER2 ) - negative , and additionally , a standard trastuzumab dose if HER2-positive .
	manualset3
206720	6	417824	7	NULL	NULL	0	NULL	capecitabine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Women with operable early-stage breast cancer were enrolled in a multicenter study of neoadjuvant therapy for four 21-day cycles with capecitabine 825mg/m ( 2 ) plus docetaxel 75mg/m ( 2 ) if human epidermal growth factor receptor 2 ( HER2 ) - negative , and additionally , a standard trastuzumab dose if HER2-positive .
	manualset3
206721	7	417824	7	NULL	NULL	NULL	NULL	 825mg/m	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Women with operable early-stage breast cancer were enrolled in a multicenter study of neoadjuvant therapy for four 21-day cycles with capecitabine 825mg/m ( 2 ) plus docetaxel 75mg/m ( 2 ) if human epidermal growth factor receptor 2 ( HER2 ) - negative , and additionally , a standard trastuzumab dose if HER2-positive .
	manualset3
206723	8	417824	7	NULL	NULL	0	NULL	docetaxel 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Women with operable early-stage breast cancer were enrolled in a multicenter study of neoadjuvant therapy for four 21-day cycles with capecitabine 825mg/m ( 2 ) plus docetaxel 75mg/m ( 2 ) if human epidermal growth factor receptor 2 ( HER2 ) - negative , and additionally , a standard trastuzumab dose if HER2-positive .
	manualset3
206725	9	417824	7	NULL	NULL	0	NULL	75mg/m	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Women with operable early-stage breast cancer were enrolled in a multicenter study of neoadjuvant therapy for four 21-day cycles with capecitabine 825mg/m ( 2 ) plus docetaxel 75mg/m ( 2 ) if human epidermal growth factor receptor 2 ( HER2 ) - negative , and additionally , a standard trastuzumab dose if HER2-positive .
	manualset3
206728	10	417824	7	NULL	NULL	NULL	NULL	human epidermal growth factor receptor 2 ( HER2 )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Women with operable early-stage breast cancer were enrolled in a multicenter study of neoadjuvant therapy for four 21-day cycles with capecitabine 825mg/m ( 2 ) plus docetaxel 75mg/m ( 2 ) if human epidermal growth factor receptor 2 ( HER2 ) - negative , and additionally , a standard trastuzumab dose if HER2-positive .
	manualset3
206730	11	417824	7	NULL	NULL	0	NULL	trastuzumab 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Women with operable early-stage breast cancer were enrolled in a multicenter study of neoadjuvant therapy for four 21-day cycles with capecitabine 825mg/m ( 2 ) plus docetaxel 75mg/m ( 2 ) if human epidermal growth factor receptor 2 ( HER2 ) - negative , and additionally , a standard trastuzumab dose if HER2-positive .
	manualset3
206732	12	417824	7	NULL	NULL	0	NULL	HER2-positive 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Women with operable early-stage breast cancer were enrolled in a multicenter study of neoadjuvant therapy for four 21-day cycles with capecitabine 825mg/m ( 2 ) plus docetaxel 75mg/m ( 2 ) if human epidermal growth factor receptor 2 ( HER2 ) - negative , and additionally , a standard trastuzumab dose if HER2-positive .
	manualset3
206733	1	417825	7	NULL	NULL	0	NULL	Wood duck ( Aix sponsa ) eggs 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Wood duck ( Aix sponsa ) eggs were incubated at three ecologically relevant temperatures ( 35 , 35.9 , 37C ) .
	manualset3
206735	2	417825	7	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Wood duck ( Aix sponsa ) eggs were incubated at three ecologically relevant temperatures ( 35 , 35.9 , 37C ) .
	manualset3
206737	3	417825	7	NULL	NULL	0	NULL	temperatures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Wood duck ( Aix sponsa ) eggs were incubated at three ecologically relevant temperatures ( 35 , 35.9 , 37C ) .
	manualset3
206739	4	417825	7	NULL	NULL	NULL	NULL	35C	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Wood duck ( Aix sponsa ) eggs were incubated at three ecologically relevant temperatures ( 35 , 35.9 , 37C ) .
	manualset3
206740	5	417825	7	NULL	NULL	0	NULL	35.9C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Wood duck ( Aix sponsa ) eggs were incubated at three ecologically relevant temperatures ( 35 , 35.9 , 37C ) .
	manualset3
206742	6	417825	7	NULL	NULL	0	NULL	37C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Wood duck ( Aix sponsa ) eggs were incubated at three ecologically relevant temperatures ( 35 , 35.9 , 37C ) .
	manualset3
206767	1	417826	7	NULL	NULL	0	NULL	Wooden picket	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Wooden picket was removed after enlarging the entry and exit wounds .
	manualset3
206768	2	417826	7	NULL	NULL	0	NULL	entry wounds	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Wooden picket was removed after enlarging the entry and exit wounds .
	manualset3
206769	3	417826	7	NULL	NULL	0	NULL	exit wounds	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Wooden picket was removed after enlarging the entry and exit wounds .
	manualset3
206770	1	417827	7	NULL	NULL	0	NULL	subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All subjects had elevated 24-h urinary levels of 18-oxo-cortisol ( 34.3 + / - 11.2 nmol/mmol creatinine ; normal range , 0.8-6 .5 nmol/mmol creatinine ) .
	manualset3
206771	2	417827	7	NULL	NULL	0	NULL	24-h urinary levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All subjects had elevated 24-h urinary levels of 18-oxo-cortisol ( 34.3 + / - 11.2 nmol/mmol creatinine ; normal range , 0.8-6 .5 nmol/mmol creatinine ) .
	manualset3
206772	3	417827	7	NULL	NULL	0	NULL	18-oxo-cortisol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All subjects had elevated 24-h urinary levels of 18-oxo-cortisol ( 34.3 + / - 11.2 nmol/mmol creatinine ; normal range , 0.8-6 .5 nmol/mmol creatinine ) .
	manualset3
206773	4	417827	7	NULL	NULL	0	NULL	34.3 + / - 11.2 nmol/mmol 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	All subjects had elevated 24-h urinary levels of 18-oxo-cortisol ( 34.3 + / - 11.2 nmol/mmol creatinine ; normal range , 0.8-6 .5 nmol/mmol creatinine ) .
	manualset3
206774	5	417827	7	NULL	NULL	0	NULL	creatinine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All subjects had elevated 24-h urinary levels of 18-oxo-cortisol ( 34.3 + / - 11.2 nmol/mmol creatinine ; normal range , 0.8-6 .5 nmol/mmol creatinine ) .
	manualset3
206775	6	417827	7	NULL	NULL	0	NULL	normal range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All subjects had elevated 24-h urinary levels of 18-oxo-cortisol ( 34.3 + / - 11.2 nmol/mmol creatinine ; normal range , 0.8-6 .5 nmol/mmol creatinine ) .
	manualset3
206776	7	417827	7	NULL	NULL	0	NULL	0.8-6 .5 nmol/mmol	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	All subjects had elevated 24-h urinary levels of 18-oxo-cortisol ( 34.3 + / - 11.2 nmol/mmol creatinine ; normal range , 0.8-6 .5 nmol/mmol creatinine ) .
	manualset3
206777	8	417827	7	NULL	NULL	0	NULL	creatinine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All subjects had elevated 24-h urinary levels of 18-oxo-cortisol ( 34.3 + / - 11.2 nmol/mmol creatinine ; normal range , 0.8-6 .5 nmol/mmol creatinine ) .
	manualset3
206778	1	417828	7	NULL	NULL	0	NULL	Word processing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Word processing : a centralized approach to hospital typing needs .
	manualset3
206779	2	417828	7	NULL	NULL	0	NULL	centralized approach 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Word processing : a centralized approach to hospital typing needs .
	manualset3
206780	3	417828	7	NULL	NULL	NULL	NULL	hospital typing needs	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Word processing : a centralized approach to hospital typing needs .
	manualset3
206781	1	417829	7	NULL	NULL	0	NULL	Words	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Words interact with colors in a globally aphasic patient : evidence from a Stroop-like task .
	manualset3
206782	2	417829	7	NULL	NULL	0	NULL	colors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Words interact with colors in a globally aphasic patient : evidence from a Stroop-like task .
	manualset3
206783	3	417829	7	NULL	NULL	0	NULL	globally aphasic patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Words interact with colors in a globally aphasic patient : evidence from a Stroop-like task .
	manualset3
206784	4	417829	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Words interact with colors in a globally aphasic patient : evidence from a Stroop-like task .
	manualset3
206785	5	417829	7	NULL	NULL	0	NULL	Stroop-like task	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Words interact with colors in a globally aphasic patient : evidence from a Stroop-like task .
	manualset3
206786	1	417830	7	NULL	NULL	0	NULL	Work characteristics 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Work characteristics ( job complexity and control ) were positively related to remaining opportunities and moderated the relationship between age and remaining opportunities , such that the relationship became weaker with increasing levels of job complexity and control .
	manualset3
206787	2	417830	7	NULL	NULL	0	NULL	 job complexity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Work characteristics ( job complexity and control ) were positively related to remaining opportunities and moderated the relationship between age and remaining opportunities , such that the relationship became weaker with increasing levels of job complexity and control .
	manualset3
206788	3	417830	7	NULL	NULL	0	NULL	control 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Work characteristics ( job complexity and control ) were positively related to remaining opportunities and moderated the relationship between age and remaining opportunities , such that the relationship became weaker with increasing levels of job complexity and control .
	manualset3
206789	4	417830	7	NULL	NULL	0	NULL	opportunities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Work characteristics ( job complexity and control ) were positively related to remaining opportunities and moderated the relationship between age and remaining opportunities , such that the relationship became weaker with increasing levels of job complexity and control .
	manualset3
206790	5	417830	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Work characteristics ( job complexity and control ) were positively related to remaining opportunities and moderated the relationship between age and remaining opportunities , such that the relationship became weaker with increasing levels of job complexity and control .
	manualset3
206791	6	417830	7	NULL	NULL	0	NULL	age	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Work characteristics ( job complexity and control ) were positively related to remaining opportunities and moderated the relationship between age and remaining opportunities , such that the relationship became weaker with increasing levels of job complexity and control .
	manualset3
206792	7	417830	7	NULL	NULL	0	NULL	opportunities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Work characteristics ( job complexity and control ) were positively related to remaining opportunities and moderated the relationship between age and remaining opportunities , such that the relationship became weaker with increasing levels of job complexity and control .
	manualset3
206793	8	417830	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Work characteristics ( job complexity and control ) were positively related to remaining opportunities and moderated the relationship between age and remaining opportunities , such that the relationship became weaker with increasing levels of job complexity and control .
	manualset3
206794	9	417830	7	NULL	NULL	0	NULL	 increasing levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Work characteristics ( job complexity and control ) were positively related to remaining opportunities and moderated the relationship between age and remaining opportunities , such that the relationship became weaker with increasing levels of job complexity and control .
	manualset3
206795	10	417830	7	NULL	NULL	0	NULL	job complexity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Work characteristics ( job complexity and control ) were positively related to remaining opportunities and moderated the relationship between age and remaining opportunities , such that the relationship became weaker with increasing levels of job complexity and control .
	manualset3
206796	11	417830	7	NULL	NULL	0	NULL	control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Work characteristics ( job complexity and control ) were positively related to remaining opportunities and moderated the relationship between age and remaining opportunities , such that the relationship became weaker with increasing levels of job complexity and control .
	manualset3
207030	1	417831	7	NULL	NULL	0	NULL	Work disability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Work disability in an inception cohort of patients with seropositive rheumatoid arthritis : a 20 year study .
	manualset3
207031	2	417831	7	NULL	NULL	0	NULL	inception cohort 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Work disability in an inception cohort of patients with seropositive rheumatoid arthritis : a 20 year study .
	manualset3
207032	3	417831	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Work disability in an inception cohort of patients with seropositive rheumatoid arthritis : a 20 year study .
	manualset3
207033	4	417831	7	NULL	NULL	0	NULL	seropositive rheumatoid arthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Work disability in an inception cohort of patients with seropositive rheumatoid arthritis : a 20 year study .
	manualset3
207034	5	417831	7	NULL	NULL	0	NULL	20 year study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Work disability in an inception cohort of patients with seropositive rheumatoid arthritis : a 20 year study .
	manualset3
207035	1	417832	7	NULL	NULL	0	NULL	Work	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Work has concentrated on the mechanisms by which abscisic acid ( ABA ) induces changes in specific ion channels at both the plasmalemma and the tonoplast , leading to efflux of both K + and anions at both membranes , requiring four essential changes .
	manualset3
207036	2	417832	7	NULL	NULL	0	NULL	mechanisms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Work has concentrated on the mechanisms by which abscisic acid ( ABA ) induces changes in specific ion channels at both the plasmalemma and the tonoplast , leading to efflux of both K + and anions at both membranes , requiring four essential changes .
	manualset3
207037	3	417832	7	NULL	NULL	0	NULL	abscisic acid ( ABA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Work has concentrated on the mechanisms by which abscisic acid ( ABA ) induces changes in specific ion channels at both the plasmalemma and the tonoplast , leading to efflux of both K + and anions at both membranes , requiring four essential changes .
	manualset3
207038	4	417832	7	NULL	NULL	0	NULL	changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Work has concentrated on the mechanisms by which abscisic acid ( ABA ) induces changes in specific ion channels at both the plasmalemma and the tonoplast , leading to efflux of both K + and anions at both membranes , requiring four essential changes .
	manualset3
207039	5	417832	7	NULL	NULL	0	NULL	specific ion channels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Work has concentrated on the mechanisms by which abscisic acid ( ABA ) induces changes in specific ion channels at both the plasmalemma and the tonoplast , leading to efflux of both K + and anions at both membranes , requiring four essential changes .
	manualset3
207040	6	417832	7	NULL	NULL	0	NULL	plasmalemma	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Work has concentrated on the mechanisms by which abscisic acid ( ABA ) induces changes in specific ion channels at both the plasmalemma and the tonoplast , leading to efflux of both K + and anions at both membranes , requiring four essential changes .
	manualset3
207041	7	417832	7	NULL	NULL	0	NULL	tonoplast	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Work has concentrated on the mechanisms by which abscisic acid ( ABA ) induces changes in specific ion channels at both the plasmalemma and the tonoplast , leading to efflux of both K + and anions at both membranes , requiring four essential changes .
	manualset3
207042	8	417832	7	NULL	NULL	0	NULL	K + 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Work has concentrated on the mechanisms by which abscisic acid ( ABA ) induces changes in specific ion channels at both the plasmalemma and the tonoplast , leading to efflux of both K + and anions at both membranes , requiring four essential changes .
	manualset3
207043	9	417832	7	NULL	NULL	0	NULL	 anions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Work has concentrated on the mechanisms by which abscisic acid ( ABA ) induces changes in specific ion channels at both the plasmalemma and the tonoplast , leading to efflux of both K + and anions at both membranes , requiring four essential changes .
	manualset3
207044	10	417832	7	NULL	NULL	0	NULL	membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Work has concentrated on the mechanisms by which abscisic acid ( ABA ) induces changes in specific ion channels at both the plasmalemma and the tonoplast , leading to efflux of both K + and anions at both membranes , requiring four essential changes .
	manualset3
207045	11	417832	7	NULL	NULL	0	NULL	 four essential changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Work has concentrated on the mechanisms by which abscisic acid ( ABA ) induces changes in specific ion channels at both the plasmalemma and the tonoplast , leading to efflux of both K + and anions at both membranes , requiring four essential changes .
	manualset3
207046	1	417833	7	NULL	NULL	0	NULL	Work	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Work involving constant movement is a risk and may lead to premature delivery .
	manualset3
207047	2	417833	7	NULL	NULL	0	NULL	constant movement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Work involving constant movement is a risk and may lead to premature delivery .
	manualset3
207048	3	417833	7	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Work involving constant movement is a risk and may lead to premature delivery .
	manualset3
207049	4	417833	7	NULL	NULL	0	NULL	premature delivery	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Work involving constant movement is a risk and may lead to premature delivery .
	manualset3
207050	1	417834	7	NULL	NULL	0	NULL	Working	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Working with an impaired team member Key words : impaired health care provider , substance abuse , patient advocate .
	manualset3
207051	2	417834	7	NULL	NULL	0	NULL	impaired team member	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Working with an impaired team member Key words : impaired health care provider , substance abuse , patient advocate .
	manualset3
207052	3	417834	7	NULL	NULL	0	NULL	Key words	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Working with an impaired team member Key words : impaired health care provider , substance abuse , patient advocate .
	manualset3
207053	4	417834	7	NULL	NULL	0	NULL	 impaired health care provider	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Working with an impaired team member Key words : impaired health care provider , substance abuse , patient advocate .
	manualset3
207054	5	417834	7	NULL	NULL	0	NULL	substance abuse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Working with an impaired team member Key words : impaired health care provider , substance abuse , patient advocate .
	manualset3
207055	6	417834	7	NULL	NULL	0	NULL	patient advocate	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Working with an impaired team member Key words : impaired health care provider , substance abuse , patient advocate .
	manualset3
207104	1	417835	7	NULL	NULL	0	NULL	subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All subjects underwent assessments of physical fitness ( aerobic capacity , back strength , and flexibility ) and EMG PS analysis of the multifidus and iliocostalis muscles ( during a constant force contraction ) , before and after the experimental period .
	manualset3
207107	2	417835	7	NULL	NULL	0	NULL	assessments	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All subjects underwent assessments of physical fitness ( aerobic capacity , back strength , and flexibility ) and EMG PS analysis of the multifidus and iliocostalis muscles ( during a constant force contraction ) , before and after the experimental period .
	manualset3
207108	3	417835	7	NULL	NULL	0	NULL	physical fitness 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All subjects underwent assessments of physical fitness ( aerobic capacity , back strength , and flexibility ) and EMG PS analysis of the multifidus and iliocostalis muscles ( during a constant force contraction ) , before and after the experimental period .
	manualset3
207109	4	417835	7	NULL	NULL	0	NULL	aerobic capacity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All subjects underwent assessments of physical fitness ( aerobic capacity , back strength , and flexibility ) and EMG PS analysis of the multifidus and iliocostalis muscles ( during a constant force contraction ) , before and after the experimental period .
	manualset3
207110	5	417835	7	NULL	NULL	0	NULL	back strength	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All subjects underwent assessments of physical fitness ( aerobic capacity , back strength , and flexibility ) and EMG PS analysis of the multifidus and iliocostalis muscles ( during a constant force contraction ) , before and after the experimental period .
	manualset3
207111	6	417835	7	NULL	NULL	0	NULL	flexibility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All subjects underwent assessments of physical fitness ( aerobic capacity , back strength , and flexibility ) and EMG PS analysis of the multifidus and iliocostalis muscles ( during a constant force contraction ) , before and after the experimental period .
	manualset3
207112	7	417835	7	NULL	NULL	0	NULL	 EMG PS analysis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All subjects underwent assessments of physical fitness ( aerobic capacity , back strength , and flexibility ) and EMG PS analysis of the multifidus and iliocostalis muscles ( during a constant force contraction ) , before and after the experimental period .
	manualset3
207113	8	417835	7	NULL	NULL	0	NULL	multifidus muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	All subjects underwent assessments of physical fitness ( aerobic capacity , back strength , and flexibility ) and EMG PS analysis of the multifidus and iliocostalis muscles ( during a constant force contraction ) , before and after the experimental period .
	manualset3
207114	9	417835	7	NULL	NULL	0	NULL	 iliocostalis muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	All subjects underwent assessments of physical fitness ( aerobic capacity , back strength , and flexibility ) and EMG PS analysis of the multifidus and iliocostalis muscles ( during a constant force contraction ) , before and after the experimental period .
	manualset3
207115	10	417835	7	NULL	NULL	0	NULL	constant force contraction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	All subjects underwent assessments of physical fitness ( aerobic capacity , back strength , and flexibility ) and EMG PS analysis of the multifidus and iliocostalis muscles ( during a constant force contraction ) , before and after the experimental period .
	manualset3
207116	11	417835	7	NULL	NULL	0	NULL	experimental period	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	All subjects underwent assessments of physical fitness ( aerobic capacity , back strength , and flexibility ) and EMG PS analysis of the multifidus and iliocostalis muscles ( during a constant force contraction ) , before and after the experimental period .
	manualset3
207117	1	417836	7	NULL	NULL	0	NULL	WormBook 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	WormBook represents a generic publishing infrastructure that is easily adaptable to other research communities to facilitate the dissemination of knowledge in the field .
	manualset3
207118	2	417836	7	NULL	NULL	0	NULL	generic publishing infrastructure	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	WormBook represents a generic publishing infrastructure that is easily adaptable to other research communities to facilitate the dissemination of knowledge in the field .
	manualset3
207119	3	417836	7	NULL	NULL	0	NULL	 research communities	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	WormBook represents a generic publishing infrastructure that is easily adaptable to other research communities to facilitate the dissemination of knowledge in the field .
	manualset3
207120	4	417836	7	NULL	NULL	0	NULL	dissemination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	WormBook represents a generic publishing infrastructure that is easily adaptable to other research communities to facilitate the dissemination of knowledge in the field .
	manualset3
207121	5	417836	7	NULL	NULL	0	NULL	knowledge	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	WormBook represents a generic publishing infrastructure that is easily adaptable to other research communities to facilitate the dissemination of knowledge in the field .
	manualset3
207122	6	417836	7	NULL	NULL	0	NULL	field	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	WormBook represents a generic publishing infrastructure that is easily adaptable to other research communities to facilitate the dissemination of knowledge in the field .
	manualset3
207123	1	417837	7	NULL	NULL	NULL	NULL	Wound epithelium	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Wound epithelium thickened when recombinant newt FGF-1 was provided on heparin-coated beads , demonstrating that the FGF-1 was biologically active and that the wound epithelium is a possible target tissue of FGF .
	manualset3
207124	2	417837	7	NULL	NULL	NULL	NULL	recombinant new FGF-1 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Wound epithelium thickened when recombinant newt FGF-1 was provided on heparin-coated beads , demonstrating that the FGF-1 was biologically active and that the wound epithelium is a possible target tissue of FGF .
	manualset3
207125	3	417837	7	NULL	NULL	0	NULL	heparin-coated beads	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Wound epithelium thickened when recombinant newt FGF-1 was provided on heparin-coated beads , demonstrating that the FGF-1 was biologically active and that the wound epithelium is a possible target tissue of FGF .
	manualset3
207126	4	417837	7	NULL	NULL	0	NULL	FGF-1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Wound epithelium thickened when recombinant newt FGF-1 was provided on heparin-coated beads , demonstrating that the FGF-1 was biologically active and that the wound epithelium is a possible target tissue of FGF .
	manualset3
207127	5	417837	7	NULL	NULL	0	NULL	wound epithelium	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Wound epithelium thickened when recombinant newt FGF-1 was provided on heparin-coated beads , demonstrating that the FGF-1 was biologically active and that the wound epithelium is a possible target tissue of FGF .
	manualset3
207128	6	417837	7	NULL	NULL	0	NULL	 tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Wound epithelium thickened when recombinant newt FGF-1 was provided on heparin-coated beads , demonstrating that the FGF-1 was biologically active and that the wound epithelium is a possible target tissue of FGF .
	manualset3
207129	7	417837	7	NULL	NULL	0	NULL	FGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Wound epithelium thickened when recombinant newt FGF-1 was provided on heparin-coated beads , demonstrating that the FGF-1 was biologically active and that the wound epithelium is a possible target tissue of FGF .
	manualset3
207130	1	417838	7	NULL	NULL	0	NULL	Wound healing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Wound healing was assessed by measurement of the breaking strengths of wound samples .
	manualset3
207131	2	417838	7	NULL	NULL	0	NULL	measurement	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Wound healing was assessed by measurement of the breaking strengths of wound samples .
	manualset3
207132	3	417838	7	NULL	NULL	0	NULL	 breaking strengths	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Wound healing was assessed by measurement of the breaking strengths of wound samples .
	manualset3
207133	4	417838	7	NULL	NULL	0	NULL	wound samples	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Wound healing was assessed by measurement of the breaking strengths of wound samples .
	manualset3
207134	1	417839	7	NULL	NULL	0	NULL	Wound healing complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Wound healing complications with de novo sirolimus versus mycophenolate mofetil-based regimen in cardiac transplant recipients .
	manualset3
207135	2	417839	7	NULL	NULL	0	NULL	de novo sirolimus	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Wound healing complications with de novo sirolimus versus mycophenolate mofetil-based regimen in cardiac transplant recipients .
	manualset3
207136	3	417839	7	NULL	NULL	0	NULL	mycophenolate mofetil-based regimen	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Wound healing complications with de novo sirolimus versus mycophenolate mofetil-based regimen in cardiac transplant recipients .
	manualset3
207137	4	417839	7	NULL	NULL	0	NULL	cardiac transplant recipients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Wound healing complications with de novo sirolimus versus mycophenolate mofetil-based regimen in cardiac transplant recipients .
	manualset3
207138	1	417840	7	NULL	NULL	0	NULL	Wound management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Wound management : are you getting it right ?
	manualset3
207139	1	417841	7	NULL	NULL	0	NULL	Writing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Writing for international publication in nursing journals : a personal perspective ( part 1 ) .
	manualset3
207140	2	417841	7	NULL	NULL	0	NULL	international publication	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Writing for international publication in nursing journals : a personal perspective ( part 1 ) .
	manualset3
207141	3	417841	7	NULL	NULL	0	NULL	 nursing journals	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Writing for international publication in nursing journals : a personal perspective ( part 1 ) .
	manualset3
207142	4	417841	7	NULL	NULL	0	NULL	 personal perspective	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Writing for international publication in nursing journals : a personal perspective ( part 1 ) .
	manualset3
207143	5	417841	7	NULL	NULL	0	NULL	part 1	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Writing for international publication in nursing journals : a personal perspective ( part 1 ) .
	manualset3
207144	1	417842	7	NULL	NULL	0	NULL	Wyeth	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Wyeth and Ligand entered into a discovery research collaboration for bazedoxifene in September 1994 .
	manualset3
207145	2	417842	7	NULL	NULL	0	NULL	Ligand	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Wyeth and Ligand entered into a discovery research collaboration for bazedoxifene in September 1994 .
	manualset3
207146	3	417842	7	NULL	NULL	0	NULL	discovery research collaboration	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Wyeth and Ligand entered into a discovery research collaboration for bazedoxifene in September 1994 .
	manualset3
207147	4	417842	7	NULL	NULL	0	NULL	bazedoxifene	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Wyeth and Ligand entered into a discovery research collaboration for bazedoxifene in September 1994 .
	manualset3
207148	5	417842	7	NULL	NULL	0	NULL	September 1994 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Wyeth and Ligand entered into a discovery research collaboration for bazedoxifene in September 1994 .
	manualset3
207149	1	417843	7	NULL	NULL	0	NULL	X-ray absorption near-edge spectroscopy measurements	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray absorption near-edge spectroscopy measurements showed only Cr ( III ) bound predominantly to formate and acetate ligands , in the bulk and rhizosphere soils , respectively .
	manualset3
207150	2	417843	7	NULL	NULL	0	NULL	Cr ( III )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray absorption near-edge spectroscopy measurements showed only Cr ( III ) bound predominantly to formate and acetate ligands , in the bulk and rhizosphere soils , respectively .
	manualset3
207151	3	417843	7	NULL	NULL	0	NULL	formate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray absorption near-edge spectroscopy measurements showed only Cr ( III ) bound predominantly to formate and acetate ligands , in the bulk and rhizosphere soils , respectively .
	manualset3
207152	4	417843	7	NULL	NULL	0	NULL	acetate ligands	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray absorption near-edge spectroscopy measurements showed only Cr ( III ) bound predominantly to formate and acetate ligands , in the bulk and rhizosphere soils , respectively .
	manualset3
207153	5	417843	7	NULL	NULL	0	NULL	bulk soils	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray absorption near-edge spectroscopy measurements showed only Cr ( III ) bound predominantly to formate and acetate ligands , in the bulk and rhizosphere soils , respectively .
	manualset3
207154	6	417843	7	NULL	NULL	0	NULL	rhizosphere soils	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray absorption near-edge spectroscopy measurements showed only Cr ( III ) bound predominantly to formate and acetate ligands , in the bulk and rhizosphere soils , respectively .
	manualset3
207155	1	417844	7	NULL	NULL	0	NULL	X-ray crystal analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray crystal analysis revealed that 1a , 1b , 2a , and 3 have triangular M ( 3 ) S ( 2 ) core structures .
	manualset3
207156	2	417844	7	NULL	NULL	0	NULL	1a 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray crystal analysis revealed that 1a , 1b , 2a , and 3 have triangular M ( 3 ) S ( 2 ) core structures .
	manualset3
207157	3	417844	7	NULL	NULL	0	NULL	1b	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray crystal analysis revealed that 1a , 1b , 2a , and 3 have triangular M ( 3 ) S ( 2 ) core structures .
	manualset3
207158	4	417844	7	NULL	NULL	0	NULL	2a 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray crystal analysis revealed that 1a , 1b , 2a , and 3 have triangular M ( 3 ) S ( 2 ) core structures .
	manualset3
207159	5	417844	7	NULL	NULL	0	NULL	3	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray crystal analysis revealed that 1a , 1b , 2a , and 3 have triangular M ( 3 ) S ( 2 ) core structures .
	manualset3
207160	6	417844	7	NULL	NULL	0	NULL	 triangular M ( 3 ) S ( 2 ) core structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray crystal analysis revealed that 1a , 1b , 2a , and 3 have triangular M ( 3 ) S ( 2 ) core structures .
	manualset3
207161	1	417845	7	NULL	NULL	0	NULL	X-ray crystallographic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray crystallographic analysis of these ( Et ( 4 ) N ) ( 2 ) ( MoEL ( 2 ) ) ( E = terminal chalocogenide ) complexes reveals an isostructural Mo center that adopts a distorted square pyramidal geometry .
	manualset3
207162	2	417845	7	NULL	NULL	0	NULL	( Et ( 4 ) N ) ( 2 ) ( MoEL ( 2 ) ) ( E = terminal chalocogenide ) complexes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray crystallographic analysis of these ( Et ( 4 ) N ) ( 2 ) ( MoEL ( 2 ) ) ( E = terminal chalocogenide ) complexes reveals an isostructural Mo center that adopts a distorted square pyramidal geometry .
	manualset3
207163	3	417845	7	NULL	NULL	0	NULL	isostructural Mo center	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray crystallographic analysis of these ( Et ( 4 ) N ) ( 2 ) ( MoEL ( 2 ) ) ( E = terminal chalocogenide ) complexes reveals an isostructural Mo center that adopts a distorted square pyramidal geometry .
	manualset3
207164	4	417845	7	NULL	NULL	0	NULL	distorted square pyramidal geometry	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray crystallographic analysis of these ( Et ( 4 ) N ) ( 2 ) ( MoEL ( 2 ) ) ( E = terminal chalocogenide ) complexes reveals an isostructural Mo center that adopts a distorted square pyramidal geometry .
	manualset3
207165	1	417846	7	NULL	NULL	0	NULL	X-ray structure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray structure of HI0817 from Haemophilus influenzae : protein of unknown function with a novel fold .
	manualset3
207166	2	417846	7	NULL	NULL	0	NULL	HI0817	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray structure of HI0817 from Haemophilus influenzae : protein of unknown function with a novel fold .
	manualset3
207167	3	417846	7	NULL	NULL	0	NULL	Haemophilus influenzae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray structure of HI0817 from Haemophilus influenzae : protein of unknown function with a novel fold .
	manualset3
207168	4	417846	7	NULL	NULL	0	NULL	protein	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray structure of HI0817 from Haemophilus influenzae : protein of unknown function with a novel fold .
	manualset3
207169	5	417846	7	NULL	NULL	0	NULL	unknown function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray structure of HI0817 from Haemophilus influenzae : protein of unknown function with a novel fold .
	manualset3
207170	6	417846	7	NULL	NULL	0	NULL	novel fold	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray structure of HI0817 from Haemophilus influenzae : protein of unknown function with a novel fold .
	manualset3
207171	1	417847	7	NULL	NULL	0	NULL	X-ray studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray studies of 7a , 5b , and 5c give insight into the origin of enantioselection and the sense of asymmetric induction in the previously reported asymmetric Diels-Alder and Ficini cycloaddition reactions with 2 , 3-disubstituted butadienes and ynamides , respectively .
	manualset3
207172	2	417847	7	NULL	NULL	0	NULL	7a	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray studies of 7a , 5b , and 5c give insight into the origin of enantioselection and the sense of asymmetric induction in the previously reported asymmetric Diels-Alder and Ficini cycloaddition reactions with 2 , 3-disubstituted butadienes and ynamides , respectively .
	manualset3
207173	3	417847	7	NULL	NULL	0	NULL	5b	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray studies of 7a , 5b , and 5c give insight into the origin of enantioselection and the sense of asymmetric induction in the previously reported asymmetric Diels-Alder and Ficini cycloaddition reactions with 2 , 3-disubstituted butadienes and ynamides , respectively .
	manualset3
207174	4	417847	7	NULL	NULL	0	NULL	5c	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray studies of 7a , 5b , and 5c give insight into the origin of enantioselection and the sense of asymmetric induction in the previously reported asymmetric Diels-Alder and Ficini cycloaddition reactions with 2 , 3-disubstituted butadienes and ynamides , respectively .
	manualset3
207175	5	417847	7	NULL	NULL	0	NULL	origin	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray studies of 7a , 5b , and 5c give insight into the origin of enantioselection and the sense of asymmetric induction in the previously reported asymmetric Diels-Alder and Ficini cycloaddition reactions with 2 , 3-disubstituted butadienes and ynamides , respectively .
	manualset3
207176	6	417847	7	NULL	NULL	0	NULL	enantioselection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray studies of 7a , 5b , and 5c give insight into the origin of enantioselection and the sense of asymmetric induction in the previously reported asymmetric Diels-Alder and Ficini cycloaddition reactions with 2 , 3-disubstituted butadienes and ynamides , respectively .
	manualset3
207177	7	417847	7	NULL	NULL	0	NULL	 sense	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray studies of 7a , 5b , and 5c give insight into the origin of enantioselection and the sense of asymmetric induction in the previously reported asymmetric Diels-Alder and Ficini cycloaddition reactions with 2 , 3-disubstituted butadienes and ynamides , respectively .
	manualset3
207178	8	417847	7	NULL	NULL	0	NULL	asymmetric induction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray studies of 7a , 5b , and 5c give insight into the origin of enantioselection and the sense of asymmetric induction in the previously reported asymmetric Diels-Alder and Ficini cycloaddition reactions with 2 , 3-disubstituted butadienes and ynamides , respectively .
	manualset3
207179	9	417847	7	NULL	NULL	0	NULL	asymmetric Diels-Alder reactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray studies of 7a , 5b , and 5c give insight into the origin of enantioselection and the sense of asymmetric induction in the previously reported asymmetric Diels-Alder and Ficini cycloaddition reactions with 2 , 3-disubstituted butadienes and ynamides , respectively .
	manualset3
207180	10	417847	7	NULL	NULL	0	NULL	Ficini cycloaddition reactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray studies of 7a , 5b , and 5c give insight into the origin of enantioselection and the sense of asymmetric induction in the previously reported asymmetric Diels-Alder and Ficini cycloaddition reactions with 2 , 3-disubstituted butadienes and ynamides , respectively .
	manualset3
207181	11	417847	7	NULL	NULL	0	NULL	2 , 3-disubstituted butadienes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray studies of 7a , 5b , and 5c give insight into the origin of enantioselection and the sense of asymmetric induction in the previously reported asymmetric Diels-Alder and Ficini cycloaddition reactions with 2 , 3-disubstituted butadienes and ynamides , respectively .
	manualset3
207182	12	417847	7	NULL	NULL	0	NULL	ynamides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray studies of 7a , 5b , and 5c give insight into the origin of enantioselection and the sense of asymmetric induction in the previously reported asymmetric Diels-Alder and Ficini cycloaddition reactions with 2 , 3-disubstituted butadienes and ynamides , respectively .
	manualset3
207183	1	417848	7	NULL	NULL	0	NULL	X chromosome inactivation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	X chromosome inactivation is unique among dosage compensation mechanisms in that the two X chromosomes in females are treated differently within the same cell ; one X chromosome is stably silenced while the other remains active .
	manualset3
207184	2	417848	7	NULL	NULL	0	NULL	dosage compensation mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	X chromosome inactivation is unique among dosage compensation mechanisms in that the two X chromosomes in females are treated differently within the same cell ; one X chromosome is stably silenced while the other remains active .
	manualset3
207185	3	417848	7	NULL	NULL	0	NULL	two X chromosomes	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	X chromosome inactivation is unique among dosage compensation mechanisms in that the two X chromosomes in females are treated differently within the same cell ; one X chromosome is stably silenced while the other remains active .
	manualset3
207186	4	417848	7	NULL	NULL	0	NULL	females	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	X chromosome inactivation is unique among dosage compensation mechanisms in that the two X chromosomes in females are treated differently within the same cell ; one X chromosome is stably silenced while the other remains active .
	manualset3
207187	5	417848	7	NULL	NULL	0	NULL	cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	X chromosome inactivation is unique among dosage compensation mechanisms in that the two X chromosomes in females are treated differently within the same cell ; one X chromosome is stably silenced while the other remains active .
	manualset3
207188	6	417848	7	NULL	NULL	0	NULL	one X chromosome	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	X chromosome inactivation is unique among dosage compensation mechanisms in that the two X chromosomes in females are treated differently within the same cell ; one X chromosome is stably silenced while the other remains active .
	manualset3
207189	1	417849	7	NULL	NULL	0	NULL	Xanthine oxidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Xanthine oxidase uses oxygen to oxidize hypoxanthine to xanthine to uric acid .
	manualset3
207190	2	417849	7	NULL	NULL	0	NULL	oxygen	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Xanthine oxidase uses oxygen to oxidize hypoxanthine to xanthine to uric acid .
	manualset3
207191	3	417849	7	NULL	NULL	0	NULL	hypoxanthine	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Xanthine oxidase uses oxygen to oxidize hypoxanthine to xanthine to uric acid .
	manualset3
207192	4	417849	7	NULL	NULL	0	NULL	 xanthine	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Xanthine oxidase uses oxygen to oxidize hypoxanthine to xanthine to uric acid .
	manualset3
207193	5	417849	7	NULL	NULL	0	NULL	uric acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Xanthine oxidase uses oxygen to oxidize hypoxanthine to xanthine to uric acid .
	manualset3
207194	1	417850	7	NULL	NULL	0	NULL	Xenobiotic compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Xenobiotic compounds accumulate in activated sludge resulting from wastewater treatment plants serving both civil and industrial areas .
	manualset3
207195	2	417850	7	NULL	NULL	0	NULL	activated sludge	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Xenobiotic compounds accumulate in activated sludge resulting from wastewater treatment plants serving both civil and industrial areas .
	manualset3
207196	3	417850	7	NULL	NULL	0	NULL	wastewater treatment plants	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Xenobiotic compounds accumulate in activated sludge resulting from wastewater treatment plants serving both civil and industrial areas .
	manualset3
207197	4	417850	7	NULL	NULL	0	NULL	civil areas	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Xenobiotic compounds accumulate in activated sludge resulting from wastewater treatment plants serving both civil and industrial areas .
	manualset3
207198	5	417850	7	NULL	NULL	0	NULL	industrial areas	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Xenobiotic compounds accumulate in activated sludge resulting from wastewater treatment plants serving both civil and industrial areas .
	manualset3
207199	1	417851	7	NULL	NULL	0	NULL	Xrcc2 ( - / - ) embryos	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Xrcc2 ( - / - ) embryos surviving until later stages of embryogenesis commonly showed developmental abnormalities and died at birth .
	manualset3
207200	2	417851	7	NULL	NULL	0	NULL	later stages	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Xrcc2 ( - / - ) embryos surviving until later stages of embryogenesis commonly showed developmental abnormalities and died at birth .
	manualset3
207201	3	417851	7	NULL	NULL	0	NULL	embryogenesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Xrcc2 ( - / - ) embryos surviving until later stages of embryogenesis commonly showed developmental abnormalities and died at birth .
	manualset3
207202	4	417851	7	NULL	NULL	0	NULL	developmental abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Xrcc2 ( - / - ) embryos surviving until later stages of embryogenesis commonly showed developmental abnormalities and died at birth .
	manualset3
207203	5	417851	7	NULL	NULL	0	NULL	birth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Xrcc2 ( - / - ) embryos surviving until later stages of embryogenesis commonly showed developmental abnormalities and died at birth .
	manualset3
207204	1	417852	7	NULL	NULL	0	NULL	Xrs2p	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Xrs2p regulates Mre11p translocation to the nucleus and plays a role in telomere elongation and meiotic recombination .
	manualset3
207205	2	417852	7	NULL	NULL	0	NULL	Mre11p	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Xrs2p regulates Mre11p translocation to the nucleus and plays a role in telomere elongation and meiotic recombination .
	manualset3
207206	3	417852	7	NULL	NULL	0	NULL	translocation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Xrs2p regulates Mre11p translocation to the nucleus and plays a role in telomere elongation and meiotic recombination .
	manualset3
207207	4	417852	7	NULL	NULL	0	NULL	 nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Xrs2p regulates Mre11p translocation to the nucleus and plays a role in telomere elongation and meiotic recombination .
	manualset3
207208	5	417852	7	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Xrs2p regulates Mre11p translocation to the nucleus and plays a role in telomere elongation and meiotic recombination .
	manualset3
207209	6	417852	7	NULL	NULL	0	NULL	telomere elongation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Xrs2p regulates Mre11p translocation to the nucleus and plays a role in telomere elongation and meiotic recombination .
	manualset3
207210	7	417852	7	NULL	NULL	0	NULL	meiotic recombination 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Xrs2p regulates Mre11p translocation to the nucleus and plays a role in telomere elongation and meiotic recombination .
	manualset3
207211	1	417853	7	NULL	NULL	0	NULL	Y-chromosome polymorphism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Y-chromosome polymorphism using short tandem repeat ( STR ) markers on 94 normal males belonging to the Brahmin and Kamma caste populations of Andhra Pradesh , India , and Siddis , a migrant population from Africa , inhabiting Hyderabad , India , revealed heterogeneity as indicated by network analysis .
	manualset3
207212	2	417853	7	NULL	NULL	0	NULL	short tandem repeat ( STR ) markers	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Y-chromosome polymorphism using short tandem repeat ( STR ) markers on 94 normal males belonging to the Brahmin and Kamma caste populations of Andhra Pradesh , India , and Siddis , a migrant population from Africa , inhabiting Hyderabad , India , revealed heterogeneity as indicated by network analysis .
	manualset3
207213	3	417853	7	NULL	NULL	0	NULL	 94 normal males	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Y-chromosome polymorphism using short tandem repeat ( STR ) markers on 94 normal males belonging to the Brahmin and Kamma caste populations of Andhra Pradesh , India , and Siddis , a migrant population from Africa , inhabiting Hyderabad , India , revealed heterogeneity as indicated by network analysis .
	manualset3
207214	4	417853	7	NULL	NULL	0	NULL	 Brahmin  caste populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Y-chromosome polymorphism using short tandem repeat ( STR ) markers on 94 normal males belonging to the Brahmin and Kamma caste populations of Andhra Pradesh , India , and Siddis , a migrant population from Africa , inhabiting Hyderabad , India , revealed heterogeneity as indicated by network analysis .
	manualset3
207215	5	417853	7	NULL	NULL	0	NULL	Kamma caste populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Y-chromosome polymorphism using short tandem repeat ( STR ) markers on 94 normal males belonging to the Brahmin and Kamma caste populations of Andhra Pradesh , India , and Siddis , a migrant population from Africa , inhabiting Hyderabad , India , revealed heterogeneity as indicated by network analysis .
	manualset3
207216	6	417853	7	NULL	NULL	0	NULL	Andhra Pradesh	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Y-chromosome polymorphism using short tandem repeat ( STR ) markers on 94 normal males belonging to the Brahmin and Kamma caste populations of Andhra Pradesh , India , and Siddis , a migrant population from Africa , inhabiting Hyderabad , India , revealed heterogeneity as indicated by network analysis .
	manualset3
207217	7	417853	7	NULL	NULL	0	NULL	India	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Y-chromosome polymorphism using short tandem repeat ( STR ) markers on 94 normal males belonging to the Brahmin and Kamma caste populations of Andhra Pradesh , India , and Siddis , a migrant population from Africa , inhabiting Hyderabad , India , revealed heterogeneity as indicated by network analysis .
	manualset3
207218	8	417853	7	NULL	NULL	0	NULL	Siddis	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Y-chromosome polymorphism using short tandem repeat ( STR ) markers on 94 normal males belonging to the Brahmin and Kamma caste populations of Andhra Pradesh , India , and Siddis , a migrant population from Africa , inhabiting Hyderabad , India , revealed heterogeneity as indicated by network analysis .
	manualset3
207219	9	417853	7	NULL	NULL	0	NULL	migrant population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Y-chromosome polymorphism using short tandem repeat ( STR ) markers on 94 normal males belonging to the Brahmin and Kamma caste populations of Andhra Pradesh , India , and Siddis , a migrant population from Africa , inhabiting Hyderabad , India , revealed heterogeneity as indicated by network analysis .
	manualset3
207220	10	417853	7	NULL	NULL	0	NULL	Africa	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Y-chromosome polymorphism using short tandem repeat ( STR ) markers on 94 normal males belonging to the Brahmin and Kamma caste populations of Andhra Pradesh , India , and Siddis , a migrant population from Africa , inhabiting Hyderabad , India , revealed heterogeneity as indicated by network analysis .
	manualset3
207221	11	417853	7	NULL	NULL	0	NULL	Hyderabad	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Y-chromosome polymorphism using short tandem repeat ( STR ) markers on 94 normal males belonging to the Brahmin and Kamma caste populations of Andhra Pradesh , India , and Siddis , a migrant population from Africa , inhabiting Hyderabad , India , revealed heterogeneity as indicated by network analysis .
	manualset3
207222	12	417853	7	NULL	NULL	0	NULL	 India	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Y-chromosome polymorphism using short tandem repeat ( STR ) markers on 94 normal males belonging to the Brahmin and Kamma caste populations of Andhra Pradesh , India , and Siddis , a migrant population from Africa , inhabiting Hyderabad , India , revealed heterogeneity as indicated by network analysis .
	manualset3
207223	13	417853	7	NULL	NULL	0	NULL	heterogeneity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Y-chromosome polymorphism using short tandem repeat ( STR ) markers on 94 normal males belonging to the Brahmin and Kamma caste populations of Andhra Pradesh , India , and Siddis , a migrant population from Africa , inhabiting Hyderabad , India , revealed heterogeneity as indicated by network analysis .
	manualset3
207224	14	417853	7	NULL	NULL	0	NULL	network analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Y-chromosome polymorphism using short tandem repeat ( STR ) markers on 94 normal males belonging to the Brahmin and Kamma caste populations of Andhra Pradesh , India , and Siddis , a migrant population from Africa , inhabiting Hyderabad , India , revealed heterogeneity as indicated by network analysis .
	manualset3
207225	1	417854	7	NULL	NULL	0	NULL	YAC-1	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	YAC-1 was less tumorigenic than A.H-2 - in normal as well as NK-depleted syngeneic A/Sn mice .
	manualset3
207226	2	417854	7	NULL	NULL	0	NULL	A.H-2 -	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	YAC-1 was less tumorigenic than A.H-2 - in normal as well as NK-depleted syngeneic A/Sn mice .
	manualset3
207227	3	417854	7	NULL	NULL	0	NULL	normal mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	YAC-1 was less tumorigenic than A.H-2 - in normal as well as NK-depleted syngeneic A/Sn mice .
	manualset3
207228	4	417854	7	NULL	NULL	0	NULL	NK-depleted syngeneic A/Sn mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	YAC-1 was less tumorigenic than A.H-2 - in normal as well as NK-depleted syngeneic A/Sn mice .
	manualset3
207229	1	417855	7	NULL	NULL	0	NULL	Critical flow levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Critical flow levels in cerebral ischemia .
	manualset3
207230	2	417855	7	NULL	NULL	0	NULL	cerebral ischemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Critical flow levels in cerebral ischemia .
	manualset3
207231	1	417856	7	NULL	NULL	0	NULL	 surveys	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	All surveys show very disappointing levels of compliance or continuance , with typically about 25 % of women stopping within 6 months and very few remaining on therapy for more than 1 or 2 years .
	manualset3
207232	2	417856	7	NULL	NULL	0	NULL	disappointing levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All surveys show very disappointing levels of compliance or continuance , with typically about 25 % of women stopping within 6 months and very few remaining on therapy for more than 1 or 2 years .
	manualset3
207233	3	417856	7	NULL	NULL	0	NULL	compliance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	All surveys show very disappointing levels of compliance or continuance , with typically about 25 % of women stopping within 6 months and very few remaining on therapy for more than 1 or 2 years .
	manualset3
207234	4	417856	7	NULL	NULL	0	NULL	continuance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	All surveys show very disappointing levels of compliance or continuance , with typically about 25 % of women stopping within 6 months and very few remaining on therapy for more than 1 or 2 years .
	manualset3
207235	5	417856	7	NULL	NULL	0	NULL	25 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All surveys show very disappointing levels of compliance or continuance , with typically about 25 % of women stopping within 6 months and very few remaining on therapy for more than 1 or 2 years .
	manualset3
207236	6	417856	7	NULL	NULL	0	NULL	women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All surveys show very disappointing levels of compliance or continuance , with typically about 25 % of women stopping within 6 months and very few remaining on therapy for more than 1 or 2 years .
	manualset3
207237	7	417856	7	NULL	NULL	0	NULL	6 months 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	All surveys show very disappointing levels of compliance or continuance , with typically about 25 % of women stopping within 6 months and very few remaining on therapy for more than 1 or 2 years .
	manualset3
207238	8	417856	7	NULL	NULL	0	NULL	 therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All surveys show very disappointing levels of compliance or continuance , with typically about 25 % of women stopping within 6 months and very few remaining on therapy for more than 1 or 2 years .
	manualset3
207239	9	417856	7	NULL	NULL	0	NULL	1 or 2 years .	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	All surveys show very disappointing levels of compliance or continuance , with typically about 25 % of women stopping within 6 months and very few remaining on therapy for more than 1 or 2 years .
	manualset3
207240	1	417857	7	NULL	NULL	0	NULL	YKL-40	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	YKL-40 is secreted by cancer cells , and elevated serum YKL-40 in patients with metastatic breast cancer and colorectal cancer is associated with a poorer prognosis as compared to patients with normal serum YKL-40 .
	manualset3
207241	2	417857	7	NULL	NULL	0	NULL	cancer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	YKL-40 is secreted by cancer cells , and elevated serum YKL-40 in patients with metastatic breast cancer and colorectal cancer is associated with a poorer prognosis as compared to patients with normal serum YKL-40 .
	manualset3
207242	3	417857	7	NULL	NULL	0	NULL	elevated serum YKL-40	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	YKL-40 is secreted by cancer cells , and elevated serum YKL-40 in patients with metastatic breast cancer and colorectal cancer is associated with a poorer prognosis as compared to patients with normal serum YKL-40 .
	manualset3
207243	4	417857	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	YKL-40 is secreted by cancer cells , and elevated serum YKL-40 in patients with metastatic breast cancer and colorectal cancer is associated with a poorer prognosis as compared to patients with normal serum YKL-40 .
	manualset3
207244	5	417857	7	NULL	NULL	0	NULL	metastatic breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	YKL-40 is secreted by cancer cells , and elevated serum YKL-40 in patients with metastatic breast cancer and colorectal cancer is associated with a poorer prognosis as compared to patients with normal serum YKL-40 .
	manualset3
207245	6	417857	7	NULL	NULL	0	NULL	colorectal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	YKL-40 is secreted by cancer cells , and elevated serum YKL-40 in patients with metastatic breast cancer and colorectal cancer is associated with a poorer prognosis as compared to patients with normal serum YKL-40 .
	manualset3
207246	7	417857	7	NULL	NULL	0	NULL	poorer prognosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	YKL-40 is secreted by cancer cells , and elevated serum YKL-40 in patients with metastatic breast cancer and colorectal cancer is associated with a poorer prognosis as compared to patients with normal serum YKL-40 .
	manualset3
207247	8	417857	7	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	YKL-40 is secreted by cancer cells , and elevated serum YKL-40 in patients with metastatic breast cancer and colorectal cancer is associated with a poorer prognosis as compared to patients with normal serum YKL-40 .
	manualset3
207248	9	417857	7	NULL	NULL	0	NULL	normal serum YKL-40	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	YKL-40 is secreted by cancer cells , and elevated serum YKL-40 in patients with metastatic breast cancer and colorectal cancer is associated with a poorer prognosis as compared to patients with normal serum YKL-40 .
	manualset3
207249	1	417858	7	NULL	NULL	0	NULL	Yawning	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Yawning is also depressed by D-amphetamine .
	manualset3
207250	2	417858	7	NULL	NULL	0	NULL	D-amphetamine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Yawning is also depressed by D-amphetamine .
	manualset3
207251	1	417859	7	NULL	NULL	0	NULL	Yeast cytochrome c messenger RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Yeast cytochrome c messenger RNA .
	manualset3
207252	1	417860	7	NULL	NULL	0	NULL	Yeast hydrolysate	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Yeast hydrolysate induces longitudinal bone growth and growth hormone release in rats .
	manualset3
207253	2	417860	7	NULL	NULL	0	NULL	longitudinal bone growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Yeast hydrolysate induces longitudinal bone growth and growth hormone release in rats .
	manualset3
207254	3	417860	7	NULL	NULL	0	NULL	growth hormone release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Yeast hydrolysate induces longitudinal bone growth and growth hormone release in rats .
	manualset3
207255	4	417860	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Yeast hydrolysate induces longitudinal bone growth and growth hormone release in rats .
	manualset3
207256	1	417861	7	NULL	NULL	0	NULL	Yellow fever vaccination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Yellow fever vaccination of primates .
	manualset3
207257	2	417861	7	NULL	NULL	0	NULL	 primates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Yellow fever vaccination of primates .
	manualset3
207258	1	417862	7	NULL	NULL	0	NULL	 no transposase sequence	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Yet no transposase sequence similar to RAG1 or RAG2 has been found .
	manualset3
207259	2	417862	7	NULL	NULL	0	NULL	RAG1	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Yet no transposase sequence similar to RAG1 or RAG2 has been found .
	manualset3
207260	3	417862	7	NULL	NULL	0	NULL	RAG2 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Yet no transposase sequence similar to RAG1 or RAG2 has been found .
	manualset3
207261	1	417863	7	NULL	NULL	0	NULL	ten patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All ten patients were at an advanced stage of oral squamous cell carcinoma ( SCC , Stage IVA , IVB or IVC ) .
	manualset3
207262	2	417863	7	NULL	NULL	0	NULL	advanced stage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All ten patients were at an advanced stage of oral squamous cell carcinoma ( SCC , Stage IVA , IVB or IVC ) .
	manualset3
207263	3	417863	7	NULL	NULL	0	NULL	oral squamous cell carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	All ten patients were at an advanced stage of oral squamous cell carcinoma ( SCC , Stage IVA , IVB or IVC ) .
	manualset3
207264	4	417863	7	NULL	NULL	0	NULL	 SCC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	All ten patients were at an advanced stage of oral squamous cell carcinoma ( SCC , Stage IVA , IVB or IVC ) .
	manualset3
207265	5	417863	7	NULL	NULL	0	NULL	Stage IVA	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All ten patients were at an advanced stage of oral squamous cell carcinoma ( SCC , Stage IVA , IVB or IVC ) .
	manualset3
207266	6	417863	7	NULL	NULL	0	NULL	IVB	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All ten patients were at an advanced stage of oral squamous cell carcinoma ( SCC , Stage IVA , IVB or IVC ) .
	manualset3
207267	7	417863	7	NULL	NULL	0	NULL	IVC	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All ten patients were at an advanced stage of oral squamous cell carcinoma ( SCC , Stage IVA , IVB or IVC ) .
	manualset3
207268	1	417864	7	NULL	NULL	0	NULL	 significance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Yet the significance of AAPB relative to total bacteria ( AAPB % ) in different marine regimes are still controversial , and variation trend of genetic diversity of AAPB along environmental gradients remains unclear .
	manualset3
207269	2	417864	7	NULL	NULL	0	NULL	AAPB	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Yet the significance of AAPB relative to total bacteria ( AAPB % ) in different marine regimes are still controversial , and variation trend of genetic diversity of AAPB along environmental gradients remains unclear .
	manualset3
207270	3	417864	7	NULL	NULL	0	NULL	 total bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Yet the significance of AAPB relative to total bacteria ( AAPB % ) in different marine regimes are still controversial , and variation trend of genetic diversity of AAPB along environmental gradients remains unclear .
	manualset3
207271	4	417864	7	NULL	NULL	0	NULL	 AAPB %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Yet the significance of AAPB relative to total bacteria ( AAPB % ) in different marine regimes are still controversial , and variation trend of genetic diversity of AAPB along environmental gradients remains unclear .
	manualset3
207272	5	417864	7	NULL	NULL	0	NULL	marine regimes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Yet the significance of AAPB relative to total bacteria ( AAPB % ) in different marine regimes are still controversial , and variation trend of genetic diversity of AAPB along environmental gradients remains unclear .
	manualset3
207273	6	417864	7	NULL	NULL	NULL	NULL	variation trend	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Yet the significance of AAPB relative to total bacteria ( AAPB % ) in different marine regimes are still controversial , and variation trend of genetic diversity of AAPB along environmental gradients remains unclear .
	manualset3
207274	7	417864	7	NULL	NULL	0	NULL	genetic diversity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Yet the significance of AAPB relative to total bacteria ( AAPB % ) in different marine regimes are still controversial , and variation trend of genetic diversity of AAPB along environmental gradients remains unclear .
	manualset3
207275	8	417864	7	NULL	NULL	0	NULL	AAPB 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Yet the significance of AAPB relative to total bacteria ( AAPB % ) in different marine regimes are still controversial , and variation trend of genetic diversity of AAPB along environmental gradients remains unclear .
	manualset3
207276	9	417864	7	NULL	NULL	0	NULL	environmental gradients	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Yet the significance of AAPB relative to total bacteria ( AAPB % ) in different marine regimes are still controversial , and variation trend of genetic diversity of AAPB along environmental gradients remains unclear .
	manualset3
207277	1	417865	7	NULL	NULL	0	NULL	successful	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Yet those who are successful in achieving such operational tolerance ( no immunosuppression and normal allograft function ) are considered lucky .
	manualset3
207278	2	417865	7	NULL	NULL	0	NULL	operational tolerance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Yet those who are successful in achieving such operational tolerance ( no immunosuppression and normal allograft function ) are considered lucky .
	manualset3
207279	3	417865	7	NULL	NULL	0	NULL	 immunosuppression 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Yet those who are successful in achieving such operational tolerance ( no immunosuppression and normal allograft function ) are considered lucky .
	manualset3
207280	4	417865	7	NULL	NULL	0	NULL	normal allograft function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Yet those who are successful in achieving such operational tolerance ( no immunosuppression and normal allograft function ) are considered lucky .
	manualset3
207281	1	417866	7	NULL	NULL	0	NULL	Yield	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Yield and purity of 82Sr produced via the natRb ( p , xn ) 82Sr process .
	manualset3
207282	2	417866	7	NULL	NULL	0	NULL	purity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Yield and purity of 82Sr produced via the natRb ( p , xn ) 82Sr process .
	manualset3
207283	3	417866	7	NULL	NULL	0	NULL	82Sr	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Yield and purity of 82Sr produced via the natRb ( p , xn ) 82Sr process .
	manualset3
207284	4	417866	7	NULL	NULL	0	NULL	natRb ( p , xn ) 82Sr process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Yield and purity of 82Sr produced via the natRb ( p , xn ) 82Sr process .
	manualset3
207285	1	417867	7	NULL	NULL	0	NULL	Young age patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Young age patients who present themselves late and delay in the initiation of anti-tuberculous therapy correlated significantly with poor outcome .
	manualset3
207286	2	417867	7	NULL	NULL	0	NULL	initiation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Young age patients who present themselves late and delay in the initiation of anti-tuberculous therapy correlated significantly with poor outcome .
	manualset3
207287	3	417867	7	NULL	NULL	0	NULL	anti-tuberculous therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Young age patients who present themselves late and delay in the initiation of anti-tuberculous therapy correlated significantly with poor outcome .
	manualset3
207288	4	417867	7	NULL	NULL	0	NULL	poor outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Young age patients who present themselves late and delay in the initiation of anti-tuberculous therapy correlated significantly with poor outcome .
	manualset3
207289	1	417868	7	NULL	NULL	0	NULL	Young endothelial cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Young endothelial cells proliferating along the endothelial basement membrane , which remained around the thrombi , and recanalization were observed on the 7th day .
	manualset3
207290	2	417868	7	NULL	NULL	0	NULL	endothelial basement membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Young endothelial cells proliferating along the endothelial basement membrane , which remained around the thrombi , and recanalization were observed on the 7th day .
	manualset3
207291	3	417868	7	NULL	NULL	0	NULL	thrombi	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Young endothelial cells proliferating along the endothelial basement membrane , which remained around the thrombi , and recanalization were observed on the 7th day .
	manualset3
207292	4	417868	7	NULL	NULL	0	NULL	recanalization 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Young endothelial cells proliferating along the endothelial basement membrane , which remained around the thrombi , and recanalization were observed on the 7th day .
	manualset3
207293	5	417868	7	NULL	NULL	0	NULL	7th day	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Young endothelial cells proliferating along the endothelial basement membrane , which remained around the thrombi , and recanalization were observed on the 7th day .
	manualset3
207294	1	417869	7	NULL	NULL	0	NULL	Young adults ' experiences	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Young adults ' experiences with cancer : comments from patients and survivors .
	manualset3
207295	2	417869	7	NULL	NULL	0	NULL	cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Young adults ' experiences with cancer : comments from patients and survivors .
	manualset3
207296	3	417869	7	NULL	NULL	0	NULL	comments	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Young adults ' experiences with cancer : comments from patients and survivors .
	manualset3
207297	4	417869	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Young adults ' experiences with cancer : comments from patients and survivors .
	manualset3
207298	5	417869	7	NULL	NULL	0	NULL	 survivors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Young adults ' experiences with cancer : comments from patients and survivors .
	manualset3
207299	1	417870	7	NULL	NULL	0	NULL	Young dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Young and middle aged dogs had significantly thicker gingiva ( 1.67 + / - 0.17 mm and 1.68 + / - 0.18 mm , respectively ) compared with older dogs ( 1.54 + / - 0.16 mm ) .
	manualset3
207300	2	417870	7	NULL	NULL	0	NULL	middle aged dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Young and middle aged dogs had significantly thicker gingiva ( 1.67 + / - 0.17 mm and 1.68 + / - 0.18 mm , respectively ) compared with older dogs ( 1.54 + / - 0.16 mm ) .
	manualset3
207301	3	417870	7	NULL	NULL	0	NULL	thicker gingiva	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Young and middle aged dogs had significantly thicker gingiva ( 1.67 + / - 0.17 mm and 1.68 + / - 0.18 mm , respectively ) compared with older dogs ( 1.54 + / - 0.16 mm ) .
	manualset3
207302	4	417870	7	NULL	NULL	0	NULL	1.67 + / - 0.17 mm 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Young and middle aged dogs had significantly thicker gingiva ( 1.67 + / - 0.17 mm and 1.68 + / - 0.18 mm , respectively ) compared with older dogs ( 1.54 + / - 0.16 mm ) .
	manualset3
207303	5	417870	7	NULL	NULL	0	NULL	1.68 + / - 0.18 mm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Young and middle aged dogs had significantly thicker gingiva ( 1.67 + / - 0.17 mm and 1.68 + / - 0.18 mm , respectively ) compared with older dogs ( 1.54 + / - 0.16 mm ) .
	manualset3
207304	6	417870	7	NULL	NULL	0	NULL	older dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Young and middle aged dogs had significantly thicker gingiva ( 1.67 + / - 0.17 mm and 1.68 + / - 0.18 mm , respectively ) compared with older dogs ( 1.54 + / - 0.16 mm ) .
	manualset3
207305	7	417870	7	NULL	NULL	0	NULL	1.54 + / - 0.16 mm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Young and middle aged dogs had significantly thicker gingiva ( 1.67 + / - 0.17 mm and 1.68 + / - 0.18 mm , respectively ) compared with older dogs ( 1.54 + / - 0.16 mm ) .
	manualset3
207306	1	417871	7	NULL	NULL	0	NULL	Younger age	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Younger age at follow-up ( p & lt ; 0.0001 ) and normal ALT levels ( p & lt ; 0.0001 ) favored clearance .
	manualset3
207307	2	417871	7	NULL	NULL	0	NULL	 p & lt ; 0.0001	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Younger age at follow-up ( p & lt ; 0.0001 ) and normal ALT levels ( p & lt ; 0.0001 ) favored clearance .
	manualset3
207308	3	417871	7	NULL	NULL	0	NULL	normal ALT levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Younger age at follow-up ( p & lt ; 0.0001 ) and normal ALT levels ( p & lt ; 0.0001 ) favored clearance .
	manualset3
207309	4	417871	7	NULL	NULL	0	NULL	p & lt ; 0.0001	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Younger age at follow-up ( p & lt ; 0.0001 ) and normal ALT levels ( p & lt ; 0.0001 ) favored clearance .
	manualset3
207310	5	417871	7	NULL	NULL	0	NULL	clearance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Younger age at follow-up ( p & lt ; 0.0001 ) and normal ALT levels ( p & lt ; 0.0001 ) favored clearance .
	manualset3
207311	6	417871	7	NULL	NULL	0	NULL	follow-up	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Younger age at follow-up ( p & lt ; 0.0001 ) and normal ALT levels ( p & lt ; 0.0001 ) favored clearance .
	manualset3
207312	1	417872	7	NULL	NULL	0	NULL	academy	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Your academy : robust and responsive .
	manualset3
207313	2	417872	7	NULL	NULL	0	NULL	responsive	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Your academy : robust and responsive .
	manualset3
207314	1	417873	7	NULL	NULL	0	NULL	 transformants 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	All transformants harbouring the modified plant DNA also acquired APS-sulfotransferase activity .
	manualset3
207315	2	417873	7	NULL	NULL	0	NULL	modified plant DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	All transformants harbouring the modified plant DNA also acquired APS-sulfotransferase activity .
	manualset3
207316	3	417873	7	NULL	NULL	0	NULL	APS-sulfotransferase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All transformants harbouring the modified plant DNA also acquired APS-sulfotransferase activity .
	manualset3
207317	1	417874	7	NULL	NULL	0	NULL	financial report 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Your financial report : fact and fiction .
	manualset3
207318	2	417874	7	NULL	NULL	0	NULL	 fact 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Your financial report : fact and fiction .
	manualset3
207319	3	417874	7	NULL	NULL	0	NULL	fiction	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Your financial report : fact and fiction .
	manualset3
207320	1	417875	7	NULL	NULL	0	NULL	Z-6 cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Z-6 , Z-43 , and Z-55 cell lines constitutively produced 192 , 48 , and 78 U/ml LT , respectively , as assessed by a cytotoxicity assay and antibody neutralization .
	manualset3
207321	2	417875	7	NULL	NULL	0	NULL	Z-43 cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Z-6 , Z-43 , and Z-55 cell lines constitutively produced 192 , 48 , and 78 U/ml LT , respectively , as assessed by a cytotoxicity assay and antibody neutralization .
	manualset3
207322	3	417875	7	NULL	NULL	0	NULL	Z-55 cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Z-6 , Z-43 , and Z-55 cell lines constitutively produced 192 , 48 , and 78 U/ml LT , respectively , as assessed by a cytotoxicity assay and antibody neutralization .
	manualset3
207323	4	417875	7	NULL	NULL	0	NULL	192 U/ml LT	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Z-6 , Z-43 , and Z-55 cell lines constitutively produced 192 , 48 , and 78 U/ml LT , respectively , as assessed by a cytotoxicity assay and antibody neutralization .
	manualset3
207324	5	417875	7	NULL	NULL	0	NULL	48 U/ml LT	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Z-6 , Z-43 , and Z-55 cell lines constitutively produced 192 , 48 , and 78 U/ml LT , respectively , as assessed by a cytotoxicity assay and antibody neutralization .
	manualset3
207325	6	417875	7	NULL	NULL	0	NULL	78 U/ml LT 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Z-6 , Z-43 , and Z-55 cell lines constitutively produced 192 , 48 , and 78 U/ml LT , respectively , as assessed by a cytotoxicity assay and antibody neutralization .
	manualset3
207326	7	417875	7	NULL	NULL	0	NULL	cytotoxicity assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Z-6 , Z-43 , and Z-55 cell lines constitutively produced 192 , 48 , and 78 U/ml LT , respectively , as assessed by a cytotoxicity assay and antibody neutralization .
	manualset3
207327	8	417875	7	NULL	NULL	0	NULL	antibody neutralization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Z-6 , Z-43 , and Z-55 cell lines constitutively produced 192 , 48 , and 78 U/ml LT , respectively , as assessed by a cytotoxicity assay and antibody neutralization .
	manualset3
207328	1	417876	7	NULL	NULL	0	NULL	ZG16p	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	ZG16p is a soluble 16kDa pancreatic protein having structural similarities with plant - prism fold lectins such as the banana lectin BanLec and the jackfruit lectin jacalin .
	manualset3
207329	2	417876	7	NULL	NULL	0	NULL	 soluble16kDa pancreatic protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	ZG16p is a soluble 16kDa pancreatic protein having structural similarities with plant - prism fold lectins such as the banana lectin BanLec and the jackfruit lectin jacalin .
	manualset3
207330	3	417876	7	NULL	NULL	0	NULL	 structural similarities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	ZG16p is a soluble 16kDa pancreatic protein having structural similarities with plant - prism fold lectins such as the banana lectin BanLec and the jackfruit lectin jacalin .
	manualset3
207331	4	417876	7	NULL	NULL	0	NULL	plant - prism fold lectins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	ZG16p is a soluble 16kDa pancreatic protein having structural similarities with plant - prism fold lectins such as the banana lectin BanLec and the jackfruit lectin jacalin .
	manualset3
207332	5	417876	7	NULL	NULL	0	NULL	 banana lectin BanLec	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	ZG16p is a soluble 16kDa pancreatic protein having structural similarities with plant - prism fold lectins such as the banana lectin BanLec and the jackfruit lectin jacalin .
	manualset3
207333	6	417876	7	NULL	NULL	0	NULL	 jackfruit lectin jacalin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	ZG16p is a soluble 16kDa pancreatic protein having structural similarities with plant - prism fold lectins such as the banana lectin BanLec and the jackfruit lectin jacalin .
	manualset3
207334	1	417877	7	NULL	NULL	0	NULL	Zearalenone ( ZEN )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Zearalenone ( ZEN ) is commonly found in many food commodities and is known to cause reproductive disorders and genotoxic effects .
	manualset3
207335	2	417877	7	NULL	NULL	0	NULL	food commodities	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Zearalenone ( ZEN ) is commonly found in many food commodities and is known to cause reproductive disorders and genotoxic effects .
	manualset3
207336	3	417877	7	NULL	NULL	0	NULL	reproductive disorders 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Zearalenone ( ZEN ) is commonly found in many food commodities and is known to cause reproductive disorders and genotoxic effects .
	manualset3
207337	4	417877	7	NULL	NULL	0	NULL	genotoxic effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Zearalenone ( ZEN ) is commonly found in many food commodities and is known to cause reproductive disorders and genotoxic effects .
	manualset3
207338	1	417878	7	NULL	NULL	0	NULL	Zeolite 4A	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Zeolite 4A also inhibited alpha-melanocyte-stimulating hormone ( alpha-MSH ) - induced melanin synthesis in B16F10 cells .
	manualset3
207339	2	417878	7	NULL	NULL	0	NULL	alpha-melanocyte-stimulating hormone ( alpha-MSH ) - induced melanin synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Zeolite 4A also inhibited alpha-melanocyte-stimulating hormone ( alpha-MSH ) - induced melanin synthesis in B16F10 cells .
	manualset3
207340	3	417878	7	NULL	NULL	0	NULL	B16F10 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Zeolite 4A also inhibited alpha-melanocyte-stimulating hormone ( alpha-MSH ) - induced melanin synthesis in B16F10 cells .
	manualset3
207341	1	417879	7	NULL	NULL	0	NULL	Zero-reflectance phenomena	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Zero-reflectance phenomena at normal incidence for both TE and TM polarizations are studied .
	manualset3
207342	2	417879	7	NULL	NULL	0	NULL	normal incidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Zero-reflectance phenomena at normal incidence for both TE and TM polarizations are studied .
	manualset3
207343	3	417879	7	NULL	NULL	0	NULL	TE polarizations 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Zero-reflectance phenomena at normal incidence for both TE and TM polarizations are studied .
	manualset3
207344	4	417879	7	NULL	NULL	0	NULL	TM polarizations	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Zero-reflectance phenomena at normal incidence for both TE and TM polarizations are studied .
	manualset3
207345	1	417880	7	NULL	NULL	0	NULL	Zinc-alpha 2-glycoprotein ( Zn alpha 2gp )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc-alpha 2-glycoprotein ( Zn alpha 2gp ) is almost ubiquitous in body fluids , and its antibody labels the corresponding secretory epithelia .
	manualset3
207346	2	417880	7	NULL	NULL	0	NULL	body fluids	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc-alpha 2-glycoprotein ( Zn alpha 2gp ) is almost ubiquitous in body fluids , and its antibody labels the corresponding secretory epithelia .
	manualset3
207347	3	417880	7	NULL	NULL	0	NULL	antibody 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc-alpha 2-glycoprotein ( Zn alpha 2gp ) is almost ubiquitous in body fluids , and its antibody labels the corresponding secretory epithelia .
	manualset3
207348	4	417880	7	NULL	NULL	0	NULL	secretory epithelia	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc-alpha 2-glycoprotein ( Zn alpha 2gp ) is almost ubiquitous in body fluids , and its antibody labels the corresponding secretory epithelia .
	manualset3
207349	1	417881	7	NULL	NULL	0	NULL	Zinc	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc , a very potent inhibitor of the NMDA receptor , is active in the forced swimming test in rats and mice .
	manualset3
207350	2	417881	7	NULL	NULL	0	NULL	 inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc , a very potent inhibitor of the NMDA receptor , is active in the forced swimming test in rats and mice .
	manualset3
207351	3	417881	7	NULL	NULL	0	NULL	NMDA receptor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc , a very potent inhibitor of the NMDA receptor , is active in the forced swimming test in rats and mice .
	manualset3
207352	4	417881	7	NULL	NULL	0	NULL	forced swimming test	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc , a very potent inhibitor of the NMDA receptor , is active in the forced swimming test in rats and mice .
	manualset3
207353	5	417881	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc , a very potent inhibitor of the NMDA receptor , is active in the forced swimming test in rats and mice .
	manualset3
207354	6	417881	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc , a very potent inhibitor of the NMDA receptor , is active in the forced swimming test in rats and mice .
	manualset3
207355	1	417882	7	NULL	NULL	0	NULL	Zinc  deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc and copper deficiency in the microvillus inclusion disease .
	manualset3
207356	2	417882	7	NULL	NULL	0	NULL	copper deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc and copper deficiency in the microvillus inclusion disease .
	manualset3
207357	3	417882	7	NULL	NULL	0	NULL	microvillus inclusion disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc and copper deficiency in the microvillus inclusion disease .
	manualset3
207358	1	417883	7	NULL	NULL	0	NULL	Zinc bis ( 1 , 4-didecylbenzo ) - bis ( 2 , 3-pyrido ) porphyrazine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc bis ( 1 , 4-didecylbenzo ) - bis ( 2 , 3-pyrido ) porphyrazine reacted with dimethyl sulfate and monochloroacetic acid to produce their quaternized products and diethyl sulfate to produce the sulfo-substituted products .
	manualset3
207359	2	417883	7	NULL	NULL	0	NULL	dimethyl sulfate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc bis ( 1 , 4-didecylbenzo ) - bis ( 2 , 3-pyrido ) porphyrazine reacted with dimethyl sulfate and monochloroacetic acid to produce their quaternized products and diethyl sulfate to produce the sulfo-substituted products .
	manualset3
207360	3	417883	7	NULL	NULL	0	NULL	monochloroacetic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc bis ( 1 , 4-didecylbenzo ) - bis ( 2 , 3-pyrido ) porphyrazine reacted with dimethyl sulfate and monochloroacetic acid to produce their quaternized products and diethyl sulfate to produce the sulfo-substituted products .
	manualset3
207361	4	417883	7	NULL	NULL	0	NULL	quaternized products	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc bis ( 1 , 4-didecylbenzo ) - bis ( 2 , 3-pyrido ) porphyrazine reacted with dimethyl sulfate and monochloroacetic acid to produce their quaternized products and diethyl sulfate to produce the sulfo-substituted products .
	manualset3
207362	5	417883	7	NULL	NULL	0	NULL	diethyl sulfate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc bis ( 1 , 4-didecylbenzo ) - bis ( 2 , 3-pyrido ) porphyrazine reacted with dimethyl sulfate and monochloroacetic acid to produce their quaternized products and diethyl sulfate to produce the sulfo-substituted products .
	manualset3
207363	6	417883	7	NULL	NULL	0	NULL	sulfo-substituted products	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc bis ( 1 , 4-didecylbenzo ) - bis ( 2 , 3-pyrido ) porphyrazine reacted with dimethyl sulfate and monochloroacetic acid to produce their quaternized products and diethyl sulfate to produce the sulfo-substituted products .
	manualset3
207364	1	417884	7	NULL	NULL	0	NULL	Zinc	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc greatly stimulates the initial rate of in vitro synthesis of 5 ' , 5 ' - diadenosine tetraphosphate by sheep liver lysyl - and phenylalanyl-tRNMA synthetases .
	manualset3
207365	2	417884	7	NULL	NULL	0	NULL	initial rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc greatly stimulates the initial rate of in vitro synthesis of 5 ' , 5 ' - diadenosine tetraphosphate by sheep liver lysyl - and phenylalanyl-tRNMA synthetases .
	manualset3
207366	3	417884	7	NULL	NULL	0	NULL	in vitro synthesis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc greatly stimulates the initial rate of in vitro synthesis of 5 ' , 5 ' - diadenosine tetraphosphate by sheep liver lysyl - and phenylalanyl-tRNMA synthetases .
	manualset3
207367	4	417884	7	NULL	NULL	0	NULL	5 ' , 5 ' - diadenosine tetraphosphate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc greatly stimulates the initial rate of in vitro synthesis of 5 ' , 5 ' - diadenosine tetraphosphate by sheep liver lysyl - and phenylalanyl-tRNMA synthetases .
	manualset3
207368	5	417884	7	NULL	NULL	0	NULL	sheep liver lysyl - and phenylalanyl-tRNMA synthetases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc greatly stimulates the initial rate of in vitro synthesis of 5 ' , 5 ' - diadenosine tetraphosphate by sheep liver lysyl - and phenylalanyl-tRNMA synthetases .
	manualset3
207369	1	417885	7	NULL	NULL	0	NULL	Zinc supplementation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc supplementation to improve mucositis and dermatitis in patients after radiotherapy for head-and-neck cancers : a double-blind , randomized study .
	manualset3
207370	2	417885	7	NULL	NULL	0	NULL	mucositis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc supplementation to improve mucositis and dermatitis in patients after radiotherapy for head-and-neck cancers : a double-blind , randomized study .
	manualset3
207371	3	417885	7	NULL	NULL	0	NULL	dermatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc supplementation to improve mucositis and dermatitis in patients after radiotherapy for head-and-neck cancers : a double-blind , randomized study .
	manualset3
207372	4	417885	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc supplementation to improve mucositis and dermatitis in patients after radiotherapy for head-and-neck cancers : a double-blind , randomized study .
	manualset3
207373	5	417885	7	NULL	NULL	0	NULL	radiotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc supplementation to improve mucositis and dermatitis in patients after radiotherapy for head-and-neck cancers : a double-blind , randomized study .
	manualset3
207374	6	417885	7	NULL	NULL	0	NULL	head-and-neck cancers 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc supplementation to improve mucositis and dermatitis in patients after radiotherapy for head-and-neck cancers : a double-blind , randomized study .
	manualset3
207375	7	417885	7	NULL	NULL	0	NULL	double-blind , randomized study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Zinc supplementation to improve mucositis and dermatitis in patients after radiotherapy for head-and-neck cancers : a double-blind , randomized study .
	manualset3
207376	1	417886	7	NULL	NULL	NULL	NULL	Zip codes	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Zip codes with higher concentrations of off-premise alcohol outlets ( e.g. , convenience or liquor stores ) and proportions of Black residents had higher rates of maltreatment .
	manualset3
207377	2	417886	7	NULL	NULL	0	NULL	higher concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Zip codes with higher concentrations of off-premise alcohol outlets ( e.g. , convenience or liquor stores ) and proportions of Black residents had higher rates of maltreatment .
	manualset3
207378	3	417886	7	NULL	NULL	0	NULL	off-premise alcohol outlets	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Zip codes with higher concentrations of off-premise alcohol outlets ( e.g. , convenience or liquor stores ) and proportions of Black residents had higher rates of maltreatment .
	manualset3
207379	4	417886	7	NULL	NULL	0	NULL	convenience stores	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Zip codes with higher concentrations of off-premise alcohol outlets ( e.g. , convenience or liquor stores ) and proportions of Black residents had higher rates of maltreatment .
	manualset3
207380	5	417886	7	NULL	NULL	0	NULL	 liquor stores	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Zip codes with higher concentrations of off-premise alcohol outlets ( e.g. , convenience or liquor stores ) and proportions of Black residents had higher rates of maltreatment .
	manualset3
207381	6	417886	7	NULL	NULL	0	NULL	 proportions	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Zip codes with higher concentrations of off-premise alcohol outlets ( e.g. , convenience or liquor stores ) and proportions of Black residents had higher rates of maltreatment .
	manualset3
207382	7	417886	7	NULL	NULL	0	NULL	Black residents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Zip codes with higher concentrations of off-premise alcohol outlets ( e.g. , convenience or liquor stores ) and proportions of Black residents had higher rates of maltreatment .
	manualset3
207383	8	417886	7	NULL	NULL	0	NULL	higher rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Zip codes with higher concentrations of off-premise alcohol outlets ( e.g. , convenience or liquor stores ) and proportions of Black residents had higher rates of maltreatment .
	manualset3
207384	9	417886	7	NULL	NULL	NULL	NULL	maltreatment	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Zip codes with higher concentrations of off-premise alcohol outlets ( e.g. , convenience or liquor stores ) and proportions of Black residents had higher rates of maltreatment .
	manualset3
207385	1	417887	7	NULL	NULL	0	NULL	ZnIn2S4 film	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	ZnIn2S4 film was fabricated on Ti substrate by a two-step approach including electrodeposition and annealing .
	manualset3
207386	2	417887	7	NULL	NULL	0	NULL	Ti substrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	ZnIn2S4 film was fabricated on Ti substrate by a two-step approach including electrodeposition and annealing .
	manualset3
207387	3	417887	7	NULL	NULL	0	NULL	 two-step approach 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	ZnIn2S4 film was fabricated on Ti substrate by a two-step approach including electrodeposition and annealing .
	manualset3
207388	4	417887	7	NULL	NULL	0	NULL	electrodeposition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	ZnIn2S4 film was fabricated on Ti substrate by a two-step approach including electrodeposition and annealing .
	manualset3
207389	5	417887	7	NULL	NULL	0	NULL	annealing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	ZnIn2S4 film was fabricated on Ti substrate by a two-step approach including electrodeposition and annealing .
	manualset3
207390	1	417888	7	NULL	NULL	0	NULL	ZnT6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	ZnT6 may function in transporting the cytoplasmic zinc into the Golgi apparatus as well as the vesicular compartment , as evidenced by its overlapping intracellular localization with TGN38 and transferrin receptor in the normal rat kidney cells .
	manualset3
207391	2	417888	7	NULL	NULL	0	NULL	cytoplasmic zinc	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	ZnT6 may function in transporting the cytoplasmic zinc into the Golgi apparatus as well as the vesicular compartment , as evidenced by its overlapping intracellular localization with TGN38 and transferrin receptor in the normal rat kidney cells .
	manualset3
207392	3	417888	7	NULL	NULL	0	NULL	Golgi apparatus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	ZnT6 may function in transporting the cytoplasmic zinc into the Golgi apparatus as well as the vesicular compartment , as evidenced by its overlapping intracellular localization with TGN38 and transferrin receptor in the normal rat kidney cells .
	manualset3
207393	4	417888	7	NULL	NULL	0	NULL	vesicular compartment	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	ZnT6 may function in transporting the cytoplasmic zinc into the Golgi apparatus as well as the vesicular compartment , as evidenced by its overlapping intracellular localization with TGN38 and transferrin receptor in the normal rat kidney cells .
	manualset3
207394	5	417888	7	NULL	NULL	0	NULL	intracellular localization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	ZnT6 may function in transporting the cytoplasmic zinc into the Golgi apparatus as well as the vesicular compartment , as evidenced by its overlapping intracellular localization with TGN38 and transferrin receptor in the normal rat kidney cells .
	manualset3
207395	6	417888	7	NULL	NULL	0	NULL	TGN38 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	ZnT6 may function in transporting the cytoplasmic zinc into the Golgi apparatus as well as the vesicular compartment , as evidenced by its overlapping intracellular localization with TGN38 and transferrin receptor in the normal rat kidney cells .
	manualset3
207396	7	417888	7	NULL	NULL	0	NULL	transferrin receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	ZnT6 may function in transporting the cytoplasmic zinc into the Golgi apparatus as well as the vesicular compartment , as evidenced by its overlapping intracellular localization with TGN38 and transferrin receptor in the normal rat kidney cells .
	manualset3
207397	8	417888	7	NULL	NULL	0	NULL	normal rat kidney cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	ZnT6 may function in transporting the cytoplasmic zinc into the Golgi apparatus as well as the vesicular compartment , as evidenced by its overlapping intracellular localization with TGN38 and transferrin receptor in the normal rat kidney cells .
	manualset3
207398	1	417889	7	NULL	NULL	0	NULL	` Living stones '	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	` Living stones ' reveal alternative petal identity programs within the core eudicots .
	manualset3
207399	2	417889	7	NULL	NULL	0	NULL	petal identity programs	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	` Living stones ' reveal alternative petal identity programs within the core eudicots .
	manualset3
207400	3	417889	7	NULL	NULL	0	NULL	core eudicots	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	` Living stones ' reveal alternative petal identity programs within the core eudicots .
	manualset3
207401	1	417890	7	NULL	NULL	0	NULL	subtotal removal	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All underwent subtotal or total removal of the tumor and a shunt procedure , foowed by irradiation therapy .
	manualset3
207402	2	417890	7	NULL	NULL	0	NULL	total removal 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All underwent subtotal or total removal of the tumor and a shunt procedure , foowed by irradiation therapy .
	manualset3
207403	3	417890	7	NULL	NULL	0	NULL	 tumor	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	All underwent subtotal or total removal of the tumor and a shunt procedure , foowed by irradiation therapy .
	manualset3
207404	4	417890	7	NULL	NULL	0	NULL	shunt procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All underwent subtotal or total removal of the tumor and a shunt procedure , foowed by irradiation therapy .
	manualset3
207405	5	417890	7	NULL	NULL	0	NULL	irradiation therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All underwent subtotal or total removal of the tumor and a shunt procedure , foowed by irradiation therapy .
	manualset3
207494	1	417891	7	NULL	NULL	NULL	NULL	Subchromosomal painting	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	` Subchromosomal painting ' will allow the identification of intrachromosomal changes on the basis of DNA homology and provides a powerful method to study karyological and genomic evolution .
	manualset3
207495	2	417891	7	NULL	NULL	0	NULL	identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	` Subchromosomal painting ' will allow the identification of intrachromosomal changes on the basis of DNA homology and provides a powerful method to study karyological and genomic evolution .
	manualset3
207496	3	417891	7	NULL	NULL	0	NULL	intrachromosomal changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	` Subchromosomal painting ' will allow the identification of intrachromosomal changes on the basis of DNA homology and provides a powerful method to study karyological and genomic evolution .
	manualset3
207497	4	417891	7	NULL	NULL	0	NULL	basis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	` Subchromosomal painting ' will allow the identification of intrachromosomal changes on the basis of DNA homology and provides a powerful method to study karyological and genomic evolution .
	manualset3
207498	5	417891	7	NULL	NULL	NULL	NULL	DNA homology	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	` Subchromosomal painting ' will allow the identification of intrachromosomal changes on the basis of DNA homology and provides a powerful method to study karyological and genomic evolution .
	manualset3
207499	6	417891	7	NULL	NULL	0	NULL	powerful method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	` Subchromosomal painting ' will allow the identification of intrachromosomal changes on the basis of DNA homology and provides a powerful method to study karyological and genomic evolution .
	manualset3
207500	7	417891	7	NULL	NULL	0	NULL	karyological evolution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	` Subchromosomal painting ' will allow the identification of intrachromosomal changes on the basis of DNA homology and provides a powerful method to study karyological and genomic evolution .
	manualset3
207501	8	417891	7	NULL	NULL	0	NULL	genomic evolution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	` Subchromosomal painting ' will allow the identification of intrachromosomal changes on the basis of DNA homology and provides a powerful method to study karyological and genomic evolution .
	manualset3
207502	1	417892	7	NULL	NULL	0	NULL	`` AICLA '' controlled trial	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	`` AICLA '' controlled trial of aspirin and dipyridamole in the secondary prevention of athero-thrombotic cerebral ischemia .
	manualset3
207503	2	417892	7	NULL	NULL	0	NULL	aspirin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	`` AICLA '' controlled trial of aspirin and dipyridamole in the secondary prevention of athero-thrombotic cerebral ischemia .
	manualset3
207504	3	417892	7	NULL	NULL	0	NULL	dipyridamole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	`` AICLA '' controlled trial of aspirin and dipyridamole in the secondary prevention of athero-thrombotic cerebral ischemia .
	manualset3
207505	4	417892	7	NULL	NULL	0	NULL	secondary prevention	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	`` AICLA '' controlled trial of aspirin and dipyridamole in the secondary prevention of athero-thrombotic cerebral ischemia .
	manualset3
207506	5	417892	7	NULL	NULL	0	NULL	athero-thrombotic cerebral ischemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	`` AICLA '' controlled trial of aspirin and dipyridamole in the secondary prevention of athero-thrombotic cerebral ischemia .
	manualset3
207507	1	417893	7	NULL	NULL	NULL	NULL	`` Awakenings '' 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	`` Awakenings '' : electrocardiographic findings in central sleep apnea .
	manualset3
207508	2	417893	7	NULL	NULL	0	NULL	electrocardiographic findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Awakenings '' : electrocardiographic findings in central sleep apnea .
	manualset3
207510	3	417893	7	NULL	NULL	0	NULL	central sleep apnea	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Awakenings '' : electrocardiographic findings in central sleep apnea .
	manualset3
207514	1	417894	7	NULL	NULL	NULL	NULL	`` Corkscrew oesophagus ''	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	`` Corkscrew oesophagus '' is characterised on the basis of two case reports and attention is drawn to thoracic pain of oesophageal origin .
	manualset3
207515	2	417894	7	NULL	NULL	0	NULL	basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Corkscrew oesophagus '' is characterised on the basis of two case reports and attention is drawn to thoracic pain of oesophageal origin .
	manualset3
207518	3	417894	7	NULL	NULL	0	NULL	two case reports 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Corkscrew oesophagus '' is characterised on the basis of two case reports and attention is drawn to thoracic pain of oesophageal origin .
	manualset3
207520	4	417894	7	NULL	NULL	0	NULL	attention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Corkscrew oesophagus '' is characterised on the basis of two case reports and attention is drawn to thoracic pain of oesophageal origin .
	manualset3
207521	5	417894	7	NULL	NULL	0	NULL	thoracic pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Corkscrew oesophagus '' is characterised on the basis of two case reports and attention is drawn to thoracic pain of oesophageal origin .
	manualset3
207522	6	417894	7	NULL	NULL	0	NULL	oesophageal origin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Corkscrew oesophagus '' is characterised on the basis of two case reports and attention is drawn to thoracic pain of oesophageal origin .
	manualset3
207523	1	417895	7	NULL	NULL	0	NULL	`` Evidence mapping '' methodology	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Evidence mapping '' methodology was used to quantify the nature and distribution of the extant high-quality research into the prevention and treatment of depression in young people across psychological , medical , and other treatment domains .
	manualset3
207524	2	417895	7	NULL	NULL	NULL	NULL	nature	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	`` Evidence mapping '' methodology was used to quantify the nature and distribution of the extant high-quality research into the prevention and treatment of depression in young people across psychological , medical , and other treatment domains .
	manualset3
207526	3	417895	7	NULL	NULL	0	NULL	distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Evidence mapping '' methodology was used to quantify the nature and distribution of the extant high-quality research into the prevention and treatment of depression in young people across psychological , medical , and other treatment domains .
	manualset3
207527	4	417895	7	NULL	NULL	0	NULL	extant high-quality research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Evidence mapping '' methodology was used to quantify the nature and distribution of the extant high-quality research into the prevention and treatment of depression in young people across psychological , medical , and other treatment domains .
	manualset3
207528	5	417895	7	NULL	NULL	0	NULL	prevention	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Evidence mapping '' methodology was used to quantify the nature and distribution of the extant high-quality research into the prevention and treatment of depression in young people across psychological , medical , and other treatment domains .
	manualset3
207530	6	417895	7	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Evidence mapping '' methodology was used to quantify the nature and distribution of the extant high-quality research into the prevention and treatment of depression in young people across psychological , medical , and other treatment domains .
	manualset3
207531	7	417895	7	NULL	NULL	0	NULL	depression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Evidence mapping '' methodology was used to quantify the nature and distribution of the extant high-quality research into the prevention and treatment of depression in young people across psychological , medical , and other treatment domains .
	manualset3
207533	8	417895	7	NULL	NULL	0	NULL	young people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Evidence mapping '' methodology was used to quantify the nature and distribution of the extant high-quality research into the prevention and treatment of depression in young people across psychological , medical , and other treatment domains .
	manualset3
207535	9	417895	7	NULL	NULL	0	NULL	psychological domain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Evidence mapping '' methodology was used to quantify the nature and distribution of the extant high-quality research into the prevention and treatment of depression in young people across psychological , medical , and other treatment domains .
	manualset3
207536	10	417895	7	NULL	NULL	0	NULL	medical domain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Evidence mapping '' methodology was used to quantify the nature and distribution of the extant high-quality research into the prevention and treatment of depression in young people across psychological , medical , and other treatment domains .
	manualset3
207537	11	417895	7	NULL	NULL	0	NULL	treatment domains	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Evidence mapping '' methodology was used to quantify the nature and distribution of the extant high-quality research into the prevention and treatment of depression in young people across psychological , medical , and other treatment domains .
	manualset3
207661	1	417896	7	NULL	NULL	0	NULL	`` Five stages '' 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Five stages '' of market consolidation , clinical rationalization , and cost competitiveness .
	manualset3
207662	2	417896	7	NULL	NULL	0	NULL	market consolidation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Five stages '' of market consolidation , clinical rationalization , and cost competitiveness .
	manualset3
207663	3	417896	7	NULL	NULL	0	NULL	clinical rationalization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Five stages '' of market consolidation , clinical rationalization , and cost competitiveness .
	manualset3
207664	4	417896	7	NULL	NULL	0	NULL	cost competitiveness 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Five stages '' of market consolidation , clinical rationalization , and cost competitiveness .
	manualset3
207665	1	417897	7	NULL	NULL	0	NULL	`` Health Care in China ''	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Health Care in China '' appeared in the May 1984 issue of the journal .
	manualset3
207666	2	417897	7	NULL	NULL	0	NULL	May 1984 issue	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Health Care in China '' appeared in the May 1984 issue of the journal .
	manualset3
207667	3	417897	7	NULL	NULL	0	NULL	journal	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Health Care in China '' appeared in the May 1984 issue of the journal .
	manualset3
207668	1	417898	7	NULL	NULL	0	NULL	vectors 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	All vectors expressed the enhanced green fluorescent protein ( GFP ) to measure transgene expression .
	manualset3
207669	2	417898	7	NULL	NULL	0	NULL	enhanced green fluorescent protein ( GFP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	All vectors expressed the enhanced green fluorescent protein ( GFP ) to measure transgene expression .
	manualset3
207670	3	417898	7	NULL	NULL	0	NULL	transgene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All vectors expressed the enhanced green fluorescent protein ( GFP ) to measure transgene expression .
	manualset3
207671	1	417899	7	NULL	NULL	0	NULL	`` Low T3-syndrome '' 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Low T3-syndrome '' in acute myocardial infarction -- relationship to beta-adrenergic blockade and clinical course .
	manualset3
207672	2	417899	7	NULL	NULL	0	NULL	acute myocardial infarction 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Low T3-syndrome '' in acute myocardial infarction -- relationship to beta-adrenergic blockade and clinical course .
	manualset3
207673	3	417899	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Low T3-syndrome '' in acute myocardial infarction -- relationship to beta-adrenergic blockade and clinical course .
	manualset3
207674	4	417899	7	NULL	NULL	0	NULL	beta-adrenergic blockade	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Low T3-syndrome '' in acute myocardial infarction -- relationship to beta-adrenergic blockade and clinical course .
	manualset3
207675	5	417899	7	NULL	NULL	0	NULL	clinical course	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Low T3-syndrome '' in acute myocardial infarction -- relationship to beta-adrenergic blockade and clinical course .
	manualset3
207676	1	417900	7	NULL	NULL	NULL	NULL	`` Normal ranges ''	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	`` Normal ranges '' and aging .
	manualset3
207677	2	417900	7	NULL	NULL	0	NULL	aging	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Normal ranges '' and aging .
	manualset3
207678	1	417901	7	NULL	NULL	0	NULL	paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	`` This paper analyses the transitions between the three states of non-employment , part-time and full-time work of a sample of married women living in West Germany ... A non-parametric duration analysis shows that women have a similar attachment to full-time and part-time work in terms of survival , and that survival in non-employment is shorter than in the other two states .
	manualset3
207679	2	417901	7	NULL	NULL	0	NULL	transitions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	`` This paper analyses the transitions between the three states of non-employment , part-time and full-time work of a sample of married women living in West Germany ... A non-parametric duration analysis shows that women have a similar attachment to full-time and part-time work in terms of survival , and that survival in non-employment is shorter than in the other two states .
	manualset3
207680	3	417901	7	NULL	NULL	0	NULL	three states 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	`` This paper analyses the transitions between the three states of non-employment , part-time and full-time work of a sample of married women living in West Germany ... A non-parametric duration analysis shows that women have a similar attachment to full-time and part-time work in terms of survival , and that survival in non-employment is shorter than in the other two states .
	manualset3
207681	4	417901	7	NULL	NULL	0	NULL	non-employment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	`` This paper analyses the transitions between the three states of non-employment , part-time and full-time work of a sample of married women living in West Germany ... A non-parametric duration analysis shows that women have a similar attachment to full-time and part-time work in terms of survival , and that survival in non-employment is shorter than in the other two states .
	manualset3
207682	5	417901	7	NULL	NULL	0	NULL	part-time work	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	`` This paper analyses the transitions between the three states of non-employment , part-time and full-time work of a sample of married women living in West Germany ... A non-parametric duration analysis shows that women have a similar attachment to full-time and part-time work in terms of survival , and that survival in non-employment is shorter than in the other two states .
	manualset3
207683	6	417901	7	NULL	NULL	0	NULL	full-time work	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	`` This paper analyses the transitions between the three states of non-employment , part-time and full-time work of a sample of married women living in West Germany ... A non-parametric duration analysis shows that women have a similar attachment to full-time and part-time work in terms of survival , and that survival in non-employment is shorter than in the other two states .
	manualset3
207684	7	417901	7	NULL	NULL	NULL	NULL	sample of married women	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	`` This paper analyses the transitions between the three states of non-employment , part-time and full-time work of a sample of married women living in West Germany ... A non-parametric duration analysis shows that women have a similar attachment to full-time and part-time work in terms of survival , and that survival in non-employment is shorter than in the other two states .
	manualset3
207686	9	417901	7	NULL	NULL	0	NULL	West Germany	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	`` This paper analyses the transitions between the three states of non-employment , part-time and full-time work of a sample of married women living in West Germany ... A non-parametric duration analysis shows that women have a similar attachment to full-time and part-time work in terms of survival , and that survival in non-employment is shorter than in the other two states .
	manualset3
207687	10	417901	7	NULL	NULL	0	NULL	non-parametric duration analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	`` This paper analyses the transitions between the three states of non-employment , part-time and full-time work of a sample of married women living in West Germany ... A non-parametric duration analysis shows that women have a similar attachment to full-time and part-time work in terms of survival , and that survival in non-employment is shorter than in the other two states .
	manualset3
207688	11	417901	7	NULL	NULL	NULL	NULL	women	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	`` This paper analyses the transitions between the three states of non-employment , part-time and full-time work of a sample of married women living in West Germany ... A non-parametric duration analysis shows that women have a similar attachment to full-time and part-time work in terms of survival , and that survival in non-employment is shorter than in the other two states .
	manualset3
207689	12	417901	7	NULL	NULL	0	NULL	attachment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	`` This paper analyses the transitions between the three states of non-employment , part-time and full-time work of a sample of married women living in West Germany ... A non-parametric duration analysis shows that women have a similar attachment to full-time and part-time work in terms of survival , and that survival in non-employment is shorter than in the other two states .
	manualset3
207690	13	417901	7	NULL	NULL	0	NULL	full-time work	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	`` This paper analyses the transitions between the three states of non-employment , part-time and full-time work of a sample of married women living in West Germany ... A non-parametric duration analysis shows that women have a similar attachment to full-time and part-time work in terms of survival , and that survival in non-employment is shorter than in the other two states .
	manualset3
207691	14	417901	7	NULL	NULL	0	NULL	part-time work	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	`` This paper analyses the transitions between the three states of non-employment , part-time and full-time work of a sample of married women living in West Germany ... A non-parametric duration analysis shows that women have a similar attachment to full-time and part-time work in terms of survival , and that survival in non-employment is shorter than in the other two states .
	manualset3
207693	16	417901	7	NULL	NULL	0	NULL	survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	`` This paper analyses the transitions between the three states of non-employment , part-time and full-time work of a sample of married women living in West Germany ... A non-parametric duration analysis shows that women have a similar attachment to full-time and part-time work in terms of survival , and that survival in non-employment is shorter than in the other two states .
	manualset3
207694	17	417901	7	NULL	NULL	0	NULL	 survival 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	`` This paper analyses the transitions between the three states of non-employment , part-time and full-time work of a sample of married women living in West Germany ... A non-parametric duration analysis shows that women have a similar attachment to full-time and part-time work in terms of survival , and that survival in non-employment is shorter than in the other two states .
	manualset3
207695	18	417901	7	NULL	NULL	0	NULL	non-employment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	`` This paper analyses the transitions between the three states of non-employment , part-time and full-time work of a sample of married women living in West Germany ... A non-parametric duration analysis shows that women have a similar attachment to full-time and part-time work in terms of survival , and that survival in non-employment is shorter than in the other two states .
	manualset3
207696	19	417901	7	NULL	NULL	NULL	NULL	two states	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	`` This paper analyses the transitions between the three states of non-employment , part-time and full-time work of a sample of married women living in West Germany ... A non-parametric duration analysis shows that women have a similar attachment to full-time and part-time work in terms of survival , and that survival in non-employment is shorter than in the other two states .
	manualset3
207697	1	417902	7	NULL	NULL	0	NULL	`` Wrong way '' misdirected axons 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Wrong way '' misdirected axons were associated with misdirected SC processes and were more numerous in bridges exposed to mitomycin , but were fewer in laminin supplemented bridges .
	manualset3
207698	2	417902	7	NULL	NULL	0	NULL	misdirected SC processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Wrong way '' misdirected axons were associated with misdirected SC processes and were more numerous in bridges exposed to mitomycin , but were fewer in laminin supplemented bridges .
	manualset3
207699	3	417902	7	NULL	NULL	0	NULL	 bridges	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Wrong way '' misdirected axons were associated with misdirected SC processes and were more numerous in bridges exposed to mitomycin , but were fewer in laminin supplemented bridges .
	manualset3
207700	4	417902	7	NULL	NULL	NULL	NULL	mitomycin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	`` Wrong way '' misdirected axons were associated with misdirected SC processes and were more numerous in bridges exposed to mitomycin , but were fewer in laminin supplemented bridges .
	manualset3
207701	5	417902	7	NULL	NULL	0	NULL	 laminin supplemented bridges	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Wrong way '' misdirected axons were associated with misdirected SC processes and were more numerous in bridges exposed to mitomycin , but were fewer in laminin supplemented bridges .
	manualset3
207702	1	417903	7	NULL	NULL	0	NULL	HP 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	All were negative for HP at the end of treatment .
	manualset3
207703	2	417903	7	NULL	NULL	0	NULL	 end	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All were negative for HP at the end of treatment .
	manualset3
207704	3	417903	7	NULL	NULL	0	NULL	 treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All were negative for HP at the end of treatment .
	manualset3
207705	1	417904	7	NULL	NULL	0	NULL	result 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A better result is then obtained by the collaboration of the surgical and prosthetic teams , for the benefit of the patient .
	manualset3
207706	2	417904	7	NULL	NULL	0	NULL	collaboration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A better result is then obtained by the collaboration of the surgical and prosthetic teams , for the benefit of the patient .
	manualset3
207707	3	417904	7	NULL	NULL	0	NULL	 surgical teams	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A better result is then obtained by the collaboration of the surgical and prosthetic teams , for the benefit of the patient .
	manualset3
207708	4	417904	7	NULL	NULL	0	NULL	prosthetic teams	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A better result is then obtained by the collaboration of the surgical and prosthetic teams , for the benefit of the patient .
	manualset3
207709	5	417904	7	NULL	NULL	0	NULL	benefit	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A better result is then obtained by the collaboration of the surgical and prosthetic teams , for the benefit of the patient .
	manualset3
207710	6	417904	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A better result is then obtained by the collaboration of the surgical and prosthetic teams , for the benefit of the patient .
	manualset3
207711	1	417905	7	NULL	NULL	0	NULL	present study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : In the present study , the effects and mechanisms of CCK-8 on HCN channels were investigated by measuring mechanical contraction of smooth muscle strips and ionic channels of ICCs in murine gastric antrum .
	manualset3
207712	2	417905	7	NULL	NULL	0	NULL	effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : In the present study , the effects and mechanisms of CCK-8 on HCN channels were investigated by measuring mechanical contraction of smooth muscle strips and ionic channels of ICCs in murine gastric antrum .
	manualset3
207713	3	417905	7	NULL	NULL	0	NULL	mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : In the present study , the effects and mechanisms of CCK-8 on HCN channels were investigated by measuring mechanical contraction of smooth muscle strips and ionic channels of ICCs in murine gastric antrum .
	manualset3
207714	4	417905	7	NULL	NULL	0	NULL	 CCK-8	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : In the present study , the effects and mechanisms of CCK-8 on HCN channels were investigated by measuring mechanical contraction of smooth muscle strips and ionic channels of ICCs in murine gastric antrum .
	manualset3
207715	5	417905	7	NULL	NULL	0	NULL	HCN channels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : In the present study , the effects and mechanisms of CCK-8 on HCN channels were investigated by measuring mechanical contraction of smooth muscle strips and ionic channels of ICCs in murine gastric antrum .
	manualset3
207716	6	417905	7	NULL	NULL	0	NULL	mechanical contraction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : In the present study , the effects and mechanisms of CCK-8 on HCN channels were investigated by measuring mechanical contraction of smooth muscle strips and ionic channels of ICCs in murine gastric antrum .
	manualset3
207717	7	417905	7	NULL	NULL	0	NULL	smooth muscle strips	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : In the present study , the effects and mechanisms of CCK-8 on HCN channels were investigated by measuring mechanical contraction of smooth muscle strips and ionic channels of ICCs in murine gastric antrum .
	manualset3
207718	8	417905	7	NULL	NULL	0	NULL	 ionic channels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : In the present study , the effects and mechanisms of CCK-8 on HCN channels were investigated by measuring mechanical contraction of smooth muscle strips and ionic channels of ICCs in murine gastric antrum .
	manualset3
207719	9	417905	7	NULL	NULL	0	NULL	ICCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : In the present study , the effects and mechanisms of CCK-8 on HCN channels were investigated by measuring mechanical contraction of smooth muscle strips and ionic channels of ICCs in murine gastric antrum .
	manualset3
207720	10	417905	7	NULL	NULL	0	NULL	murine gastric antrum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : In the present study , the effects and mechanisms of CCK-8 on HCN channels were investigated by measuring mechanical contraction of smooth muscle strips and ionic channels of ICCs in murine gastric antrum .
	manualset3
207721	11	417905	7	NULL	NULL	0	NULL	Methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Methods : In the present study , the effects and mechanisms of CCK-8 on HCN channels were investigated by measuring mechanical contraction of smooth muscle strips and ionic channels of ICCs in murine gastric antrum .
	manualset3
207722	1	417906	7	NULL	NULL	0	NULL	dissociation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , a dissociation between the neuroprotective effects of deprenyl and its MAO inhibiting effects has been proposed .
	manualset3
207723	2	417906	7	NULL	NULL	0	NULL	neuroprotective effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , a dissociation between the neuroprotective effects of deprenyl and its MAO inhibiting effects has been proposed .
	manualset3
207724	3	417906	7	NULL	NULL	0	NULL	deprenyl 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , a dissociation between the neuroprotective effects of deprenyl and its MAO inhibiting effects has been proposed .
	manualset3
207725	4	417906	7	NULL	NULL	0	NULL	MAO inhibiting effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , a dissociation between the neuroprotective effects of deprenyl and its MAO inhibiting effects has been proposed .
	manualset3
207726	1	417907	7	NULL	NULL	0	NULL	Flaps	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Flaps from the leg donor site appeared to develop more extensive postoperative congestion and edema than those from the foot donor site , which had a negative effect on flap survival .
	manualset3
207727	2	417907	7	NULL	NULL	0	NULL	 leg donor site	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Flaps from the leg donor site appeared to develop more extensive postoperative congestion and edema than those from the foot donor site , which had a negative effect on flap survival .
	manualset3
207728	3	417907	7	NULL	NULL	0	NULL	postoperative congestion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Flaps from the leg donor site appeared to develop more extensive postoperative congestion and edema than those from the foot donor site , which had a negative effect on flap survival .
	manualset3
207729	4	417907	7	NULL	NULL	0	NULL	edema	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Flaps from the leg donor site appeared to develop more extensive postoperative congestion and edema than those from the foot donor site , which had a negative effect on flap survival .
	manualset3
207730	5	417907	7	NULL	NULL	0	NULL	foot donor site	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Flaps from the leg donor site appeared to develop more extensive postoperative congestion and edema than those from the foot donor site , which had a negative effect on flap survival .
	manualset3
207731	6	417907	7	NULL	NULL	0	NULL	negative effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Flaps from the leg donor site appeared to develop more extensive postoperative congestion and edema than those from the foot donor site , which had a negative effect on flap survival .
	manualset3
207732	7	417907	7	NULL	NULL	0	NULL	flap survival 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Flaps from the leg donor site appeared to develop more extensive postoperative congestion and edema than those from the foot donor site , which had a negative effect on flap survival .
	manualset3
207733	1	417908	7	NULL	NULL	0	NULL	Early-onset multifocal inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Early-onset multifocal inflammation in the transforming growth factor beta 1-null mouse is lymphocyte mediated .
	manualset3
207734	2	417908	7	NULL	NULL	0	NULL	transforming growth factor beta 1-null mouse	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Early-onset multifocal inflammation in the transforming growth factor beta 1-null mouse is lymphocyte mediated .
	manualset3
207735	1	417909	7	NULL	NULL	0	NULL	RNase protection assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	RNase protection assays from rat tissues revealed a predominant expression for IL 1R-rp2 in the lung and epididymis with lower levels detected in the testis and cerebral cortex .
	manualset3
207736	2	417909	7	NULL	NULL	0	NULL	 rat tissues 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	RNase protection assays from rat tissues revealed a predominant expression for IL 1R-rp2 in the lung and epididymis with lower levels detected in the testis and cerebral cortex .
	manualset3
207737	3	417909	7	NULL	NULL	0	NULL	predominant expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RNase protection assays from rat tissues revealed a predominant expression for IL 1R-rp2 in the lung and epididymis with lower levels detected in the testis and cerebral cortex .
	manualset3
207738	4	417909	7	NULL	NULL	0	NULL	IL 1R-rp2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	RNase protection assays from rat tissues revealed a predominant expression for IL 1R-rp2 in the lung and epididymis with lower levels detected in the testis and cerebral cortex .
	manualset3
207739	5	417909	7	NULL	NULL	0	NULL	lung	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	RNase protection assays from rat tissues revealed a predominant expression for IL 1R-rp2 in the lung and epididymis with lower levels detected in the testis and cerebral cortex .
	manualset3
207740	6	417909	7	NULL	NULL	0	NULL	epididymis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	RNase protection assays from rat tissues revealed a predominant expression for IL 1R-rp2 in the lung and epididymis with lower levels detected in the testis and cerebral cortex .
	manualset3
207741	7	417909	7	NULL	NULL	0	NULL	lower levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	RNase protection assays from rat tissues revealed a predominant expression for IL 1R-rp2 in the lung and epididymis with lower levels detected in the testis and cerebral cortex .
	manualset3
207742	8	417909	7	NULL	NULL	0	NULL	 testis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	RNase protection assays from rat tissues revealed a predominant expression for IL 1R-rp2 in the lung and epididymis with lower levels detected in the testis and cerebral cortex .
	manualset3
207743	9	417909	7	NULL	NULL	0	NULL	cerebral cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	RNase protection assays from rat tissues revealed a predominant expression for IL 1R-rp2 in the lung and epididymis with lower levels detected in the testis and cerebral cortex .
	manualset3
207744	1	417910	7	NULL	NULL	NULL	NULL	Body weight	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Body weight was monitored for at least 1 yr before , during , and after hormone treatment .
	manualset3
207745	2	417910	7	NULL	NULL	0	NULL	1 yr	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Body weight was monitored for at least 1 yr before , during , and after hormone treatment .
	manualset3
207746	3	417910	7	NULL	NULL	0	NULL	hormone treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Body weight was monitored for at least 1 yr before , during , and after hormone treatment .
	manualset3
207747	1	417911	7	NULL	NULL	0	NULL	spinal trigeminal tract 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The spinal trigeminal tract at the level of the medulla oblongata contained viral antigen in the neurons , glia and in the vascular walls , including a few endothelial cells .
	manualset3
207748	2	417911	7	NULL	NULL	0	NULL	 level	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The spinal trigeminal tract at the level of the medulla oblongata contained viral antigen in the neurons , glia and in the vascular walls , including a few endothelial cells .
	manualset3
207749	3	417911	7	NULL	NULL	0	NULL	medulla oblongata	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The spinal trigeminal tract at the level of the medulla oblongata contained viral antigen in the neurons , glia and in the vascular walls , including a few endothelial cells .
	manualset3
207750	4	417911	7	NULL	NULL	0	NULL	viral antigen	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The spinal trigeminal tract at the level of the medulla oblongata contained viral antigen in the neurons , glia and in the vascular walls , including a few endothelial cells .
	manualset3
207751	5	417911	7	NULL	NULL	0	NULL	neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The spinal trigeminal tract at the level of the medulla oblongata contained viral antigen in the neurons , glia and in the vascular walls , including a few endothelial cells .
	manualset3
207752	6	417911	7	NULL	NULL	0	NULL	glia	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The spinal trigeminal tract at the level of the medulla oblongata contained viral antigen in the neurons , glia and in the vascular walls , including a few endothelial cells .
	manualset3
207753	7	417911	7	NULL	NULL	0	NULL	vascular walls	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The spinal trigeminal tract at the level of the medulla oblongata contained viral antigen in the neurons , glia and in the vascular walls , including a few endothelial cells .
	manualset3
207754	8	417911	7	NULL	NULL	0	NULL	endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The spinal trigeminal tract at the level of the medulla oblongata contained viral antigen in the neurons , glia and in the vascular walls , including a few endothelial cells .
	manualset3
207755	1	417912	7	NULL	NULL	0	NULL	substance 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The substance led to a dose-dependent reduction of cholesterol in the serum of various species of animals such as rat , dog and marmoset .
	manualset3
207756	2	417912	7	NULL	NULL	0	NULL	dose-dependent reduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The substance led to a dose-dependent reduction of cholesterol in the serum of various species of animals such as rat , dog and marmoset .
	manualset3
207757	3	417912	7	NULL	NULL	0	NULL	cholesterol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The substance led to a dose-dependent reduction of cholesterol in the serum of various species of animals such as rat , dog and marmoset .
	manualset3
207758	4	417912	7	NULL	NULL	0	NULL	serum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The substance led to a dose-dependent reduction of cholesterol in the serum of various species of animals such as rat , dog and marmoset .
	manualset3
207759	5	417912	7	NULL	NULL	0	NULL	species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The substance led to a dose-dependent reduction of cholesterol in the serum of various species of animals such as rat , dog and marmoset .
	manualset3
207760	6	417912	7	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The substance led to a dose-dependent reduction of cholesterol in the serum of various species of animals such as rat , dog and marmoset .
	manualset3
207761	7	417912	7	NULL	NULL	0	NULL	 rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The substance led to a dose-dependent reduction of cholesterol in the serum of various species of animals such as rat , dog and marmoset .
	manualset3
207762	8	417912	7	NULL	NULL	0	NULL	dog	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The substance led to a dose-dependent reduction of cholesterol in the serum of various species of animals such as rat , dog and marmoset .
	manualset3
207763	9	417912	7	NULL	NULL	0	NULL	marmoset	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The substance led to a dose-dependent reduction of cholesterol in the serum of various species of animals such as rat , dog and marmoset .
	manualset3
207764	1	417913	7	NULL	NULL	0	NULL	heart disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	All were without significant heart disease and under forty years of age .
	manualset3
207765	2	417913	7	NULL	NULL	NULL	NULL	forty years of age	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	All were without significant heart disease and under forty years of age .
	manualset3
207767	1	417914	7	NULL	NULL	0	NULL	Blockade	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Blockade of the pre - and postjunctional effects of angiotensin in vivo with a non-peptide angiotensin receptor antagonist .
	manualset3
207768	2	417914	7	NULL	NULL	NULL	NULL	 pre-junctional effects 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Blockade of the pre - and postjunctional effects of angiotensin in vivo with a non-peptide angiotensin receptor antagonist .
	manualset3
207769	3	417914	7	NULL	NULL	0	NULL	angiotensin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Blockade of the pre - and postjunctional effects of angiotensin in vivo with a non-peptide angiotensin receptor antagonist .
	manualset3
207770	4	417914	7	NULL	NULL	0	NULL	non-peptide angiotensin receptor antagonist 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Blockade of the pre - and postjunctional effects of angiotensin in vivo with a non-peptide angiotensin receptor antagonist .
	manualset3
207771	5	417914	7	NULL	NULL	0	NULL	postjunctional effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Blockade of the pre - and postjunctional effects of angiotensin in vivo with a non-peptide angiotensin receptor antagonist .
	manualset3
207772	1	417915	7	NULL	NULL	0	NULL	HHM 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Although most features of HHM can be explained by excessive action of circulating PTHrP , decreased serum level of 1 , 25 ( OH ) ( 2 ) D and markedly suppressed bone formation found in HHM can not be explained by the action of N-terminus of PTHrP .
	manualset3
207773	2	417915	7	NULL	NULL	0	NULL	excessive action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although most features of HHM can be explained by excessive action of circulating PTHrP , decreased serum level of 1 , 25 ( OH ) ( 2 ) D and markedly suppressed bone formation found in HHM can not be explained by the action of N-terminus of PTHrP .
	manualset3
207774	3	417915	7	NULL	NULL	0	NULL	circulating PTHrP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although most features of HHM can be explained by excessive action of circulating PTHrP , decreased serum level of 1 , 25 ( OH ) ( 2 ) D and markedly suppressed bone formation found in HHM can not be explained by the action of N-terminus of PTHrP .
	manualset3
207775	4	417915	7	NULL	NULL	0	NULL	serum level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although most features of HHM can be explained by excessive action of circulating PTHrP , decreased serum level of 1 , 25 ( OH ) ( 2 ) D and markedly suppressed bone formation found in HHM can not be explained by the action of N-terminus of PTHrP .
	manualset3
207776	5	417915	7	NULL	NULL	0	NULL	1 , 25 ( OH ) ( 2 ) D	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although most features of HHM can be explained by excessive action of circulating PTHrP , decreased serum level of 1 , 25 ( OH ) ( 2 ) D and markedly suppressed bone formation found in HHM can not be explained by the action of N-terminus of PTHrP .
	manualset3
207777	6	417915	7	NULL	NULL	0	NULL	bone formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although most features of HHM can be explained by excessive action of circulating PTHrP , decreased serum level of 1 , 25 ( OH ) ( 2 ) D and markedly suppressed bone formation found in HHM can not be explained by the action of N-terminus of PTHrP .
	manualset3
207778	7	417915	7	NULL	NULL	0	NULL	HHM	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Although most features of HHM can be explained by excessive action of circulating PTHrP , decreased serum level of 1 , 25 ( OH ) ( 2 ) D and markedly suppressed bone formation found in HHM can not be explained by the action of N-terminus of PTHrP .
	manualset3
207779	8	417915	7	NULL	NULL	0	NULL	action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although most features of HHM can be explained by excessive action of circulating PTHrP , decreased serum level of 1 , 25 ( OH ) ( 2 ) D and markedly suppressed bone formation found in HHM can not be explained by the action of N-terminus of PTHrP .
	manualset3
207780	9	417915	7	NULL	NULL	0	NULL	N-terminus	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although most features of HHM can be explained by excessive action of circulating PTHrP , decreased serum level of 1 , 25 ( OH ) ( 2 ) D and markedly suppressed bone formation found in HHM can not be explained by the action of N-terminus of PTHrP .
	manualset3
207781	10	417915	7	NULL	NULL	0	NULL	PTHrP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although most features of HHM can be explained by excessive action of circulating PTHrP , decreased serum level of 1 , 25 ( OH ) ( 2 ) D and markedly suppressed bone formation found in HHM can not be explained by the action of N-terminus of PTHrP .
	manualset3
207782	1	417916	7	NULL	NULL	0	NULL	clinical study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This clinical study assessed the influence of pentoxifylline and its metabolites on steady-state serum theophylline concentrations .
	manualset3
207783	2	417916	7	NULL	NULL	0	NULL	 influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This clinical study assessed the influence of pentoxifylline and its metabolites on steady-state serum theophylline concentrations .
	manualset3
207784	3	417916	7	NULL	NULL	0	NULL	pentoxifylline	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	This clinical study assessed the influence of pentoxifylline and its metabolites on steady-state serum theophylline concentrations .
	manualset3
207785	4	417916	7	NULL	NULL	0	NULL	metabolites 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This clinical study assessed the influence of pentoxifylline and its metabolites on steady-state serum theophylline concentrations .
	manualset3
207786	5	417916	7	NULL	NULL	0	NULL	steady-state serum theophylline concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This clinical study assessed the influence of pentoxifylline and its metabolites on steady-state serum theophylline concentrations .
	manualset3
207787	1	417917	7	NULL	NULL	0	NULL	classification system	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The classification system of Kalamchi and Dawe ( 1985 ) was found to be preferable to that of Jones , Barnes and Lloyd-Roberts ( 1978 ) as a guide to prognosis and management .
	manualset3
207788	2	417917	7	NULL	NULL	NULL	NULL	Kalamchi and Dawe ( 1985 )	PublicationOrCitation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The classification system of Kalamchi and Dawe ( 1985 ) was found to be preferable to that of Jones , Barnes and Lloyd-Roberts ( 1978 ) as a guide to prognosis and management .
	manualset3
207789	3	417917	7	NULL	NULL	0	NULL	Jones , Barnes and Lloyd-Roberts ( 1978 )	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	The classification system of Kalamchi and Dawe ( 1985 ) was found to be preferable to that of Jones , Barnes and Lloyd-Roberts ( 1978 ) as a guide to prognosis and management .
	manualset3
207790	4	417917	7	NULL	NULL	NULL	NULL	prognosis	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The classification system of Kalamchi and Dawe ( 1985 ) was found to be preferable to that of Jones , Barnes and Lloyd-Roberts ( 1978 ) as a guide to prognosis and management .
	manualset3
207791	5	417917	7	NULL	NULL	0	NULL	management 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The classification system of Kalamchi and Dawe ( 1985 ) was found to be preferable to that of Jones , Barnes and Lloyd-Roberts ( 1978 ) as a guide to prognosis and management .
	manualset3
207792	1	417918	7	NULL	NULL	0	NULL	probes	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using these probes , the cryptoregiochemistry of the Delta13 desaturation involved in the biosynthesis of Thaumetopoea pityocampa sex pheromone was studied by means of kinetic isotope effect determinations .
	manualset3
207793	2	417918	7	NULL	NULL	0	NULL	cryptoregiochemistry	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using these probes , the cryptoregiochemistry of the Delta13 desaturation involved in the biosynthesis of Thaumetopoea pityocampa sex pheromone was studied by means of kinetic isotope effect determinations .
	manualset3
207794	3	417918	7	NULL	NULL	0	NULL	Delta13 desaturation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using these probes , the cryptoregiochemistry of the Delta13 desaturation involved in the biosynthesis of Thaumetopoea pityocampa sex pheromone was studied by means of kinetic isotope effect determinations .
	manualset3
207795	4	417918	7	NULL	NULL	0	NULL	biosynthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using these probes , the cryptoregiochemistry of the Delta13 desaturation involved in the biosynthesis of Thaumetopoea pityocampa sex pheromone was studied by means of kinetic isotope effect determinations .
	manualset3
207796	5	417918	7	NULL	NULL	0	NULL	Thaumetopoea pityocampa sex pheromone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using these probes , the cryptoregiochemistry of the Delta13 desaturation involved in the biosynthesis of Thaumetopoea pityocampa sex pheromone was studied by means of kinetic isotope effect determinations .
	manualset3
207798	7	417918	7	NULL	NULL	NULL	NULL	kinetic isotope effect determinations	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using these probes , the cryptoregiochemistry of the Delta13 desaturation involved in the biosynthesis of Thaumetopoea pityocampa sex pheromone was studied by means of kinetic isotope effect determinations .
	manualset3
207799	1	417919	7	NULL	NULL	0	NULL	Carbamazepine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Carbamazepine and bone mineral metabolism .
	manualset3
207800	2	417919	7	NULL	NULL	0	NULL	bone mineral metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Carbamazepine and bone mineral metabolism .
	manualset3
207801	1	417920	7	NULL	NULL	0	NULL	mechanism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To study the mechanism of action , six additional animals received an Achilles tendon injection of the inflammatory agent carrageenan alone and six received carrageenan plus growth factor .
	manualset3
207802	2	417920	7	NULL	NULL	0	NULL	action	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To study the mechanism of action , six additional animals received an Achilles tendon injection of the inflammatory agent carrageenan alone and six received carrageenan plus growth factor .
	manualset3
207803	3	417920	7	NULL	NULL	0	NULL	 six additional animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To study the mechanism of action , six additional animals received an Achilles tendon injection of the inflammatory agent carrageenan alone and six received carrageenan plus growth factor .
	manualset3
207804	4	417920	7	NULL	NULL	0	NULL	Achilles tendon injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To study the mechanism of action , six additional animals received an Achilles tendon injection of the inflammatory agent carrageenan alone and six received carrageenan plus growth factor .
	manualset3
207805	5	417920	7	NULL	NULL	0	NULL	inflammatory agent carrageenan	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	To study the mechanism of action , six additional animals received an Achilles tendon injection of the inflammatory agent carrageenan alone and six received carrageenan plus growth factor .
	manualset3
207806	6	417920	7	NULL	NULL	0	NULL	 six 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To study the mechanism of action , six additional animals received an Achilles tendon injection of the inflammatory agent carrageenan alone and six received carrageenan plus growth factor .
	manualset3
207807	7	417920	7	NULL	NULL	0	NULL	 carrageenan plus growth factor	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	To study the mechanism of action , six additional animals received an Achilles tendon injection of the inflammatory agent carrageenan alone and six received carrageenan plus growth factor .
	manualset3
207808	1	417921	7	NULL	NULL	0	NULL	surrogate end points	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It will examine surrogate end points as well as risk factors for atherosclerosis .
	manualset3
207809	2	417921	7	NULL	NULL	0	NULL	 risk factors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It will examine surrogate end points as well as risk factors for atherosclerosis .
	manualset3
207810	3	417921	7	NULL	NULL	0	NULL	atherosclerosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It will examine surrogate end points as well as risk factors for atherosclerosis .
	manualset3
207811	1	417922	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All women were counseled about a method of contraception , particularly copper T-380A , and divided into two groups : Group 1 included 226 women who preferred immediate IUD insertion , and Group 2 included 100 women who opted for interval-IUD insertion during the first menstrual cycle after abortion .
	manualset3
207812	2	417922	7	NULL	NULL	0	NULL	 method	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All women were counseled about a method of contraception , particularly copper T-380A , and divided into two groups : Group 1 included 226 women who preferred immediate IUD insertion , and Group 2 included 100 women who opted for interval-IUD insertion during the first menstrual cycle after abortion .
	manualset3
207813	3	417922	7	NULL	NULL	0	NULL	contraception	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All women were counseled about a method of contraception , particularly copper T-380A , and divided into two groups : Group 1 included 226 women who preferred immediate IUD insertion , and Group 2 included 100 women who opted for interval-IUD insertion during the first menstrual cycle after abortion .
	manualset3
207814	4	417922	7	NULL	NULL	0	NULL	copper T-380A	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	All women were counseled about a method of contraception , particularly copper T-380A , and divided into two groups : Group 1 included 226 women who preferred immediate IUD insertion , and Group 2 included 100 women who opted for interval-IUD insertion during the first menstrual cycle after abortion .
	manualset3
207815	5	417922	7	NULL	NULL	0	NULL	two groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All women were counseled about a method of contraception , particularly copper T-380A , and divided into two groups : Group 1 included 226 women who preferred immediate IUD insertion , and Group 2 included 100 women who opted for interval-IUD insertion during the first menstrual cycle after abortion .
	manualset3
207816	6	417922	7	NULL	NULL	0	NULL	Group 1	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All women were counseled about a method of contraception , particularly copper T-380A , and divided into two groups : Group 1 included 226 women who preferred immediate IUD insertion , and Group 2 included 100 women who opted for interval-IUD insertion during the first menstrual cycle after abortion .
	manualset3
207817	7	417922	7	NULL	NULL	0	NULL	226 women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All women were counseled about a method of contraception , particularly copper T-380A , and divided into two groups : Group 1 included 226 women who preferred immediate IUD insertion , and Group 2 included 100 women who opted for interval-IUD insertion during the first menstrual cycle after abortion .
	manualset3
207818	8	417922	7	NULL	NULL	0	NULL	IUD insertion 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All women were counseled about a method of contraception , particularly copper T-380A , and divided into two groups : Group 1 included 226 women who preferred immediate IUD insertion , and Group 2 included 100 women who opted for interval-IUD insertion during the first menstrual cycle after abortion .
	manualset3
207819	9	417922	7	NULL	NULL	0	NULL	Group 2	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All women were counseled about a method of contraception , particularly copper T-380A , and divided into two groups : Group 1 included 226 women who preferred immediate IUD insertion , and Group 2 included 100 women who opted for interval-IUD insertion during the first menstrual cycle after abortion .
	manualset3
207820	10	417922	7	NULL	NULL	0	NULL	100 women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All women were counseled about a method of contraception , particularly copper T-380A , and divided into two groups : Group 1 included 226 women who preferred immediate IUD insertion , and Group 2 included 100 women who opted for interval-IUD insertion during the first menstrual cycle after abortion .
	manualset3
207821	11	417922	7	NULL	NULL	0	NULL	interval-IUD insertion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All women were counseled about a method of contraception , particularly copper T-380A , and divided into two groups : Group 1 included 226 women who preferred immediate IUD insertion , and Group 2 included 100 women who opted for interval-IUD insertion during the first menstrual cycle after abortion .
	manualset3
207822	12	417922	7	NULL	NULL	0	NULL	first menstrual cycle 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All women were counseled about a method of contraception , particularly copper T-380A , and divided into two groups : Group 1 included 226 women who preferred immediate IUD insertion , and Group 2 included 100 women who opted for interval-IUD insertion during the first menstrual cycle after abortion .
	manualset3
207823	13	417922	7	NULL	NULL	0	NULL	abortion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All women were counseled about a method of contraception , particularly copper T-380A , and divided into two groups : Group 1 included 226 women who preferred immediate IUD insertion , and Group 2 included 100 women who opted for interval-IUD insertion during the first menstrual cycle after abortion .
	manualset3
207824	1	417923	7	NULL	NULL	0	NULL	ILK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We also show that ILK performs its centrosome clustering activity in a focal adhesion-independent , but centrosome-dependent , manner through the microtubule regulating proteins TACC3 and ch-TOG .
	manualset3
207825	2	417923	7	NULL	NULL	0	NULL	centrosome clustering activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We also show that ILK performs its centrosome clustering activity in a focal adhesion-independent , but centrosome-dependent , manner through the microtubule regulating proteins TACC3 and ch-TOG .
	manualset3
207826	3	417923	7	NULL	NULL	0	NULL	focal adhesion-independent manner	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We also show that ILK performs its centrosome clustering activity in a focal adhesion-independent , but centrosome-dependent , manner through the microtubule regulating proteins TACC3 and ch-TOG .
	manualset3
207827	4	417923	7	NULL	NULL	0	NULL	centrosome-dependent manner	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We also show that ILK performs its centrosome clustering activity in a focal adhesion-independent , but centrosome-dependent , manner through the microtubule regulating proteins TACC3 and ch-TOG .
	manualset3
207828	5	417923	7	NULL	NULL	0	NULL	microtubule regulating proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We also show that ILK performs its centrosome clustering activity in a focal adhesion-independent , but centrosome-dependent , manner through the microtubule regulating proteins TACC3 and ch-TOG .
	manualset3
207829	6	417923	7	NULL	NULL	0	NULL	TACC3 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We also show that ILK performs its centrosome clustering activity in a focal adhesion-independent , but centrosome-dependent , manner through the microtubule regulating proteins TACC3 and ch-TOG .
	manualset3
207830	7	417923	7	NULL	NULL	0	NULL	ch-TOG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We also show that ILK performs its centrosome clustering activity in a focal adhesion-independent , but centrosome-dependent , manner through the microtubule regulating proteins TACC3 and ch-TOG .
	manualset3
207831	1	417924	7	NULL	NULL	NULL	NULL	Three	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Three of the hybrids , with insertions at residues 125 , 180 and 200 , assembled into the trypsin-resistant oligomeric form characteristic of the wild-type protein , which suggested that these regions are not involved in TraT subunit : subunit interactions .
	manualset3
207832	2	417924	7	NULL	NULL	0	NULL	hybrids	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Three of the hybrids , with insertions at residues 125 , 180 and 200 , assembled into the trypsin-resistant oligomeric form characteristic of the wild-type protein , which suggested that these regions are not involved in TraT subunit : subunit interactions .
	manualset3
207833	3	417924	7	NULL	NULL	0	NULL	insertions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Three of the hybrids , with insertions at residues 125 , 180 and 200 , assembled into the trypsin-resistant oligomeric form characteristic of the wild-type protein , which suggested that these regions are not involved in TraT subunit : subunit interactions .
	manualset3
207834	4	417924	7	NULL	NULL	NULL	NULL	residues 125	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Three of the hybrids , with insertions at residues 125 , 180 and 200 , assembled into the trypsin-resistant oligomeric form characteristic of the wild-type protein , which suggested that these regions are not involved in TraT subunit : subunit interactions .
	manualset3
207835	5	417924	7	NULL	NULL	0	NULL	residues 180	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Three of the hybrids , with insertions at residues 125 , 180 and 200 , assembled into the trypsin-resistant oligomeric form characteristic of the wild-type protein , which suggested that these regions are not involved in TraT subunit : subunit interactions .
	manualset3
207836	6	417924	7	NULL	NULL	0	NULL	residues 200	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Three of the hybrids , with insertions at residues 125 , 180 and 200 , assembled into the trypsin-resistant oligomeric form characteristic of the wild-type protein , which suggested that these regions are not involved in TraT subunit : subunit interactions .
	manualset3
207837	7	417924	7	NULL	NULL	0	NULL	trypsin-resistant oligomeric form	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Three of the hybrids , with insertions at residues 125 , 180 and 200 , assembled into the trypsin-resistant oligomeric form characteristic of the wild-type protein , which suggested that these regions are not involved in TraT subunit : subunit interactions .
	manualset3
207838	8	417924	7	NULL	NULL	0	NULL	wild-type protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Three of the hybrids , with insertions at residues 125 , 180 and 200 , assembled into the trypsin-resistant oligomeric form characteristic of the wild-type protein , which suggested that these regions are not involved in TraT subunit : subunit interactions .
	manualset3
207839	9	417924	7	NULL	NULL	0	NULL	regions	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Three of the hybrids , with insertions at residues 125 , 180 and 200 , assembled into the trypsin-resistant oligomeric form characteristic of the wild-type protein , which suggested that these regions are not involved in TraT subunit : subunit interactions .
	manualset3
207840	10	417924	7	NULL	NULL	0	NULL	TraT subunit : subunit interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Three of the hybrids , with insertions at residues 125 , 180 and 200 , assembled into the trypsin-resistant oligomeric form characteristic of the wild-type protein , which suggested that these regions are not involved in TraT subunit : subunit interactions .
	manualset3
207841	1	417925	7	NULL	NULL	0	NULL	gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A gene for dihydrofolate reductase in a herpesvirus .
	manualset3
207842	2	417925	7	NULL	NULL	0	NULL	dihydrofolate reductase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A gene for dihydrofolate reductase in a herpesvirus .
	manualset3
207843	3	417925	7	NULL	NULL	0	NULL	herpesvirus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A gene for dihydrofolate reductase in a herpesvirus .
	manualset3
207844	1	417926	7	NULL	NULL	0	NULL	Lapatinib	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Lapatinib is a potent reversible and selective inhibitor of the tyrosine kinase domains of epidermal growth factor receptor and human epidermal growth factor receptor ( HER ) -2 that exerts its action by competitive binding to the intracellular ATP-binding site of the receptor .
	manualset3
207845	2	417926	7	NULL	NULL	0	NULL	reversible inhibitor	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Lapatinib is a potent reversible and selective inhibitor of the tyrosine kinase domains of epidermal growth factor receptor and human epidermal growth factor receptor ( HER ) -2 that exerts its action by competitive binding to the intracellular ATP-binding site of the receptor .
	manualset3
207846	3	417926	7	NULL	NULL	0	NULL	selective inhibitor	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Lapatinib is a potent reversible and selective inhibitor of the tyrosine kinase domains of epidermal growth factor receptor and human epidermal growth factor receptor ( HER ) -2 that exerts its action by competitive binding to the intracellular ATP-binding site of the receptor .
	manualset3
207847	4	417926	7	NULL	NULL	0	NULL	tyrosine kinase domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lapatinib is a potent reversible and selective inhibitor of the tyrosine kinase domains of epidermal growth factor receptor and human epidermal growth factor receptor ( HER ) -2 that exerts its action by competitive binding to the intracellular ATP-binding site of the receptor .
	manualset3
207848	5	417926	7	NULL	NULL	0	NULL	epidermal growth factor receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lapatinib is a potent reversible and selective inhibitor of the tyrosine kinase domains of epidermal growth factor receptor and human epidermal growth factor receptor ( HER ) -2 that exerts its action by competitive binding to the intracellular ATP-binding site of the receptor .
	manualset3
207849	6	417926	7	NULL	NULL	0	NULL	human epidermal growth factor receptor ( HER ) -2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lapatinib is a potent reversible and selective inhibitor of the tyrosine kinase domains of epidermal growth factor receptor and human epidermal growth factor receptor ( HER ) -2 that exerts its action by competitive binding to the intracellular ATP-binding site of the receptor .
	manualset3
207850	7	417926	7	NULL	NULL	0	NULL	action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lapatinib is a potent reversible and selective inhibitor of the tyrosine kinase domains of epidermal growth factor receptor and human epidermal growth factor receptor ( HER ) -2 that exerts its action by competitive binding to the intracellular ATP-binding site of the receptor .
	manualset3
207851	8	417926	7	NULL	NULL	0	NULL	competitive binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lapatinib is a potent reversible and selective inhibitor of the tyrosine kinase domains of epidermal growth factor receptor and human epidermal growth factor receptor ( HER ) -2 that exerts its action by competitive binding to the intracellular ATP-binding site of the receptor .
	manualset3
207852	9	417926	7	NULL	NULL	0	NULL	intracellular ATP-binding site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lapatinib is a potent reversible and selective inhibitor of the tyrosine kinase domains of epidermal growth factor receptor and human epidermal growth factor receptor ( HER ) -2 that exerts its action by competitive binding to the intracellular ATP-binding site of the receptor .
	manualset3
207853	10	417926	7	NULL	NULL	0	NULL	receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lapatinib is a potent reversible and selective inhibitor of the tyrosine kinase domains of epidermal growth factor receptor and human epidermal growth factor receptor ( HER ) -2 that exerts its action by competitive binding to the intracellular ATP-binding site of the receptor .
	manualset3
207854	1	417927	7	NULL	NULL	0	NULL	Seventeen control patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventeen control patients followed with CT studies for a mean of 9 + / - 2 months had no spontaneous remission of lesions , and in many cases the scans showed worsening during the observation period .
	manualset3
207855	2	417927	7	NULL	NULL	0	NULL	CT studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventeen control patients followed with CT studies for a mean of 9 + / - 2 months had no spontaneous remission of lesions , and in many cases the scans showed worsening during the observation period .
	manualset3
207856	3	417927	7	NULL	NULL	0	NULL	 mean 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventeen control patients followed with CT studies for a mean of 9 + / - 2 months had no spontaneous remission of lesions , and in many cases the scans showed worsening during the observation period .
	manualset3
207857	4	417927	7	NULL	NULL	0	NULL	9 + / - 2 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventeen control patients followed with CT studies for a mean of 9 + / - 2 months had no spontaneous remission of lesions , and in many cases the scans showed worsening during the observation period .
	manualset3
207858	5	417927	7	NULL	NULL	0	NULL	no spontaneous remission	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventeen control patients followed with CT studies for a mean of 9 + / - 2 months had no spontaneous remission of lesions , and in many cases the scans showed worsening during the observation period .
	manualset3
207859	6	417927	7	NULL	NULL	0	NULL	lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventeen control patients followed with CT studies for a mean of 9 + / - 2 months had no spontaneous remission of lesions , and in many cases the scans showed worsening during the observation period .
	manualset3
207860	7	417927	7	NULL	NULL	0	NULL	 cases 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventeen control patients followed with CT studies for a mean of 9 + / - 2 months had no spontaneous remission of lesions , and in many cases the scans showed worsening during the observation period .
	manualset3
207861	8	417927	7	NULL	NULL	0	NULL	scans	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventeen control patients followed with CT studies for a mean of 9 + / - 2 months had no spontaneous remission of lesions , and in many cases the scans showed worsening during the observation period .
	manualset3
207862	9	417927	7	NULL	NULL	0	NULL	 worsening	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventeen control patients followed with CT studies for a mean of 9 + / - 2 months had no spontaneous remission of lesions , and in many cases the scans showed worsening during the observation period .
	manualset3
207863	10	417927	7	NULL	NULL	0	NULL	observation period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Seventeen control patients followed with CT studies for a mean of 9 + / - 2 months had no spontaneous remission of lesions , and in many cases the scans showed worsening during the observation period .
	manualset3
207864	1	417928	7	NULL	NULL	0	NULL	 aim	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study described here was to determine the possible contribution of the acrosin activity test to routine semen analysis in enhancing the precision of the prognosis of IVF success in a group of patients in which the contribution of the egg factor to infertility was ruled out ( 20 cases ) compared to a control IVF group ( 39 cases ) .
	manualset3
207865	2	417928	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study described here was to determine the possible contribution of the acrosin activity test to routine semen analysis in enhancing the precision of the prognosis of IVF success in a group of patients in which the contribution of the egg factor to infertility was ruled out ( 20 cases ) compared to a control IVF group ( 39 cases ) .
	manualset3
207866	3	417928	7	NULL	NULL	0	NULL	contribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study described here was to determine the possible contribution of the acrosin activity test to routine semen analysis in enhancing the precision of the prognosis of IVF success in a group of patients in which the contribution of the egg factor to infertility was ruled out ( 20 cases ) compared to a control IVF group ( 39 cases ) .
	manualset3
207867	4	417928	7	NULL	NULL	0	NULL	acrosin activity test 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study described here was to determine the possible contribution of the acrosin activity test to routine semen analysis in enhancing the precision of the prognosis of IVF success in a group of patients in which the contribution of the egg factor to infertility was ruled out ( 20 cases ) compared to a control IVF group ( 39 cases ) .
	manualset3
207868	5	417928	7	NULL	NULL	0	NULL	routine semen analysis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study described here was to determine the possible contribution of the acrosin activity test to routine semen analysis in enhancing the precision of the prognosis of IVF success in a group of patients in which the contribution of the egg factor to infertility was ruled out ( 20 cases ) compared to a control IVF group ( 39 cases ) .
	manualset3
207869	6	417928	7	NULL	NULL	0	NULL	precision	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study described here was to determine the possible contribution of the acrosin activity test to routine semen analysis in enhancing the precision of the prognosis of IVF success in a group of patients in which the contribution of the egg factor to infertility was ruled out ( 20 cases ) compared to a control IVF group ( 39 cases ) .
	manualset3
207870	7	417928	7	NULL	NULL	0	NULL	prognosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study described here was to determine the possible contribution of the acrosin activity test to routine semen analysis in enhancing the precision of the prognosis of IVF success in a group of patients in which the contribution of the egg factor to infertility was ruled out ( 20 cases ) compared to a control IVF group ( 39 cases ) .
	manualset3
207871	8	417928	7	NULL	NULL	0	NULL	IVF success 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study described here was to determine the possible contribution of the acrosin activity test to routine semen analysis in enhancing the precision of the prognosis of IVF success in a group of patients in which the contribution of the egg factor to infertility was ruled out ( 20 cases ) compared to a control IVF group ( 39 cases ) .
	manualset3
207872	9	417928	7	NULL	NULL	0	NULL	group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study described here was to determine the possible contribution of the acrosin activity test to routine semen analysis in enhancing the precision of the prognosis of IVF success in a group of patients in which the contribution of the egg factor to infertility was ruled out ( 20 cases ) compared to a control IVF group ( 39 cases ) .
	manualset3
207873	10	417928	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study described here was to determine the possible contribution of the acrosin activity test to routine semen analysis in enhancing the precision of the prognosis of IVF success in a group of patients in which the contribution of the egg factor to infertility was ruled out ( 20 cases ) compared to a control IVF group ( 39 cases ) .
	manualset3
207874	11	417928	7	NULL	NULL	0	NULL	contribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study described here was to determine the possible contribution of the acrosin activity test to routine semen analysis in enhancing the precision of the prognosis of IVF success in a group of patients in which the contribution of the egg factor to infertility was ruled out ( 20 cases ) compared to a control IVF group ( 39 cases ) .
	manualset3
207875	12	417928	7	NULL	NULL	0	NULL	egg factor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study described here was to determine the possible contribution of the acrosin activity test to routine semen analysis in enhancing the precision of the prognosis of IVF success in a group of patients in which the contribution of the egg factor to infertility was ruled out ( 20 cases ) compared to a control IVF group ( 39 cases ) .
	manualset3
207876	13	417928	7	NULL	NULL	0	NULL	infertility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study described here was to determine the possible contribution of the acrosin activity test to routine semen analysis in enhancing the precision of the prognosis of IVF success in a group of patients in which the contribution of the egg factor to infertility was ruled out ( 20 cases ) compared to a control IVF group ( 39 cases ) .
	manualset3
207877	14	417928	7	NULL	NULL	0	NULL	20 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study described here was to determine the possible contribution of the acrosin activity test to routine semen analysis in enhancing the precision of the prognosis of IVF success in a group of patients in which the contribution of the egg factor to infertility was ruled out ( 20 cases ) compared to a control IVF group ( 39 cases ) .
	manualset3
207878	15	417928	7	NULL	NULL	0	NULL	control IVF group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study described here was to determine the possible contribution of the acrosin activity test to routine semen analysis in enhancing the precision of the prognosis of IVF success in a group of patients in which the contribution of the egg factor to infertility was ruled out ( 20 cases ) compared to a control IVF group ( 39 cases ) .
	manualset3
207879	16	417928	7	NULL	NULL	0	NULL	39 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim of the study described here was to determine the possible contribution of the acrosin activity test to routine semen analysis in enhancing the precision of the prognosis of IVF success in a group of patients in which the contribution of the egg factor to infertility was ruled out ( 20 cases ) compared to a control IVF group ( 39 cases ) .
	manualset3
207880	1	417929	7	NULL	NULL	0	NULL	Surviving fractions	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Surviving fractions at 2 ( SF2 ) and 10 Gy ( SF10 ) irradiations , and those at 30 and 60 min heatings at 44 degrees C ( SF30 and SF60 ) , were obtained for each clone .
	manualset3
207881	2	417929	7	NULL	NULL	NULL	NULL	2 ( SF2 ) irradiations	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Surviving fractions at 2 ( SF2 ) and 10 Gy ( SF10 ) irradiations , and those at 30 and 60 min heatings at 44 degrees C ( SF30 and SF60 ) , were obtained for each clone .
	manualset3
207882	3	417929	7	NULL	NULL	0	NULL	10 Gy ( SF10 ) irradiations	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Surviving fractions at 2 ( SF2 ) and 10 Gy ( SF10 ) irradiations , and those at 30 and 60 min heatings at 44 degrees C ( SF30 and SF60 ) , were obtained for each clone .
	manualset3
207883	4	417929	7	NULL	NULL	0	NULL	30 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Surviving fractions at 2 ( SF2 ) and 10 Gy ( SF10 ) irradiations , and those at 30 and 60 min heatings at 44 degrees C ( SF30 and SF60 ) , were obtained for each clone .
	manualset3
207884	5	417929	7	NULL	NULL	0	NULL	 60 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Surviving fractions at 2 ( SF2 ) and 10 Gy ( SF10 ) irradiations , and those at 30 and 60 min heatings at 44 degrees C ( SF30 and SF60 ) , were obtained for each clone .
	manualset3
207885	6	417929	7	NULL	NULL	0	NULL	44 degrees C 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Surviving fractions at 2 ( SF2 ) and 10 Gy ( SF10 ) irradiations , and those at 30 and 60 min heatings at 44 degrees C ( SF30 and SF60 ) , were obtained for each clone .
	manualset3
207886	7	417929	7	NULL	NULL	0	NULL	SF30	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Surviving fractions at 2 ( SF2 ) and 10 Gy ( SF10 ) irradiations , and those at 30 and 60 min heatings at 44 degrees C ( SF30 and SF60 ) , were obtained for each clone .
	manualset3
207887	8	417929	7	NULL	NULL	0	NULL	SF60	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Surviving fractions at 2 ( SF2 ) and 10 Gy ( SF10 ) irradiations , and those at 30 and 60 min heatings at 44 degrees C ( SF30 and SF60 ) , were obtained for each clone .
	manualset3
207888	9	417929	7	NULL	NULL	0	NULL	clone	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Surviving fractions at 2 ( SF2 ) and 10 Gy ( SF10 ) irradiations , and those at 30 and 60 min heatings at 44 degrees C ( SF30 and SF60 ) , were obtained for each clone .
	manualset3
207889	1	417930	7	NULL	NULL	0	NULL	serial homology	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The serial homology of arthropods , together with our ability to identify individual neurons from segment to segment , and from animal to animal , provides opportunities for studying the changes wrought by natural selection on specific neural elements when functional requirements change in different parts of the trunk .
	manualset3
207890	2	417930	7	NULL	NULL	0	NULL	arthropods	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The serial homology of arthropods , together with our ability to identify individual neurons from segment to segment , and from animal to animal , provides opportunities for studying the changes wrought by natural selection on specific neural elements when functional requirements change in different parts of the trunk .
	manualset3
207891	3	417930	7	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The serial homology of arthropods , together with our ability to identify individual neurons from segment to segment , and from animal to animal , provides opportunities for studying the changes wrought by natural selection on specific neural elements when functional requirements change in different parts of the trunk .
	manualset3
207892	4	417930	7	NULL	NULL	0	NULL	individual neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The serial homology of arthropods , together with our ability to identify individual neurons from segment to segment , and from animal to animal , provides opportunities for studying the changes wrought by natural selection on specific neural elements when functional requirements change in different parts of the trunk .
	manualset3
207893	5	417930	7	NULL	NULL	0	NULL	segment to segment	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The serial homology of arthropods , together with our ability to identify individual neurons from segment to segment , and from animal to animal , provides opportunities for studying the changes wrought by natural selection on specific neural elements when functional requirements change in different parts of the trunk .
	manualset3
207894	6	417930	7	NULL	NULL	0	NULL	animal to animal	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The serial homology of arthropods , together with our ability to identify individual neurons from segment to segment , and from animal to animal , provides opportunities for studying the changes wrought by natural selection on specific neural elements when functional requirements change in different parts of the trunk .
	manualset3
207895	7	417930	7	NULL	NULL	0	NULL	opportunities 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The serial homology of arthropods , together with our ability to identify individual neurons from segment to segment , and from animal to animal , provides opportunities for studying the changes wrought by natural selection on specific neural elements when functional requirements change in different parts of the trunk .
	manualset3
207896	8	417930	7	NULL	NULL	0	NULL	studying	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The serial homology of arthropods , together with our ability to identify individual neurons from segment to segment , and from animal to animal , provides opportunities for studying the changes wrought by natural selection on specific neural elements when functional requirements change in different parts of the trunk .
	manualset3
207897	9	417930	7	NULL	NULL	0	NULL	changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The serial homology of arthropods , together with our ability to identify individual neurons from segment to segment , and from animal to animal , provides opportunities for studying the changes wrought by natural selection on specific neural elements when functional requirements change in different parts of the trunk .
	manualset3
207898	10	417930	7	NULL	NULL	0	NULL	natural selection 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The serial homology of arthropods , together with our ability to identify individual neurons from segment to segment , and from animal to animal , provides opportunities for studying the changes wrought by natural selection on specific neural elements when functional requirements change in different parts of the trunk .
	manualset3
207899	11	417930	7	NULL	NULL	0	NULL	specific neural elements	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The serial homology of arthropods , together with our ability to identify individual neurons from segment to segment , and from animal to animal , provides opportunities for studying the changes wrought by natural selection on specific neural elements when functional requirements change in different parts of the trunk .
	manualset3
207900	12	417930	7	NULL	NULL	0	NULL	functional requirements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The serial homology of arthropods , together with our ability to identify individual neurons from segment to segment , and from animal to animal , provides opportunities for studying the changes wrought by natural selection on specific neural elements when functional requirements change in different parts of the trunk .
	manualset3
207901	13	417930	7	NULL	NULL	0	NULL	different parts of the trunk	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The serial homology of arthropods , together with our ability to identify individual neurons from segment to segment , and from animal to animal , provides opportunities for studying the changes wrought by natural selection on specific neural elements when functional requirements change in different parts of the trunk .
	manualset3
207910	1	417931	7	NULL	NULL	0	NULL	Inhibition 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of the biological action of thyroid hormones by actinomycin D and puromycin .
	manualset3
207911	2	417931	7	NULL	NULL	0	NULL	biological action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of the biological action of thyroid hormones by actinomycin D and puromycin .
	manualset3
207912	3	417931	7	NULL	NULL	0	NULL	thyroid hormones	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of the biological action of thyroid hormones by actinomycin D and puromycin .
	manualset3
207913	4	417931	7	NULL	NULL	0	NULL	actinomycin D	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of the biological action of thyroid hormones by actinomycin D and puromycin .
	manualset3
207914	5	417931	7	NULL	NULL	0	NULL	puromycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of the biological action of thyroid hormones by actinomycin D and puromycin .
	manualset3
207915	1	417932	7	NULL	NULL	0	NULL	January 1970	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Between January 1970 and December 1982 , seventy-one patients in functional Stage IV of the NYHA classification underwent isolated aortic valve replacement for aortic incompetence ( 27 cases ) , aortic stenosis ( 18 cases ) or mixed aortic valve disease ( 26 cases ) .
	manualset3
207916	2	417932	7	NULL	NULL	0	NULL	December 1982	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Between January 1970 and December 1982 , seventy-one patients in functional Stage IV of the NYHA classification underwent isolated aortic valve replacement for aortic incompetence ( 27 cases ) , aortic stenosis ( 18 cases ) or mixed aortic valve disease ( 26 cases ) .
	manualset3
207917	3	417932	7	NULL	NULL	0	NULL	seventy-one patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Between January 1970 and December 1982 , seventy-one patients in functional Stage IV of the NYHA classification underwent isolated aortic valve replacement for aortic incompetence ( 27 cases ) , aortic stenosis ( 18 cases ) or mixed aortic valve disease ( 26 cases ) .
	manualset3
207918	4	417932	7	NULL	NULL	NULL	NULL	functional Stage IV	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between January 1970 and December 1982 , seventy-one patients in functional Stage IV of the NYHA classification underwent isolated aortic valve replacement for aortic incompetence ( 27 cases ) , aortic stenosis ( 18 cases ) or mixed aortic valve disease ( 26 cases ) .
	manualset3
207919	5	417932	7	NULL	NULL	0	NULL	NYHA classification	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Between January 1970 and December 1982 , seventy-one patients in functional Stage IV of the NYHA classification underwent isolated aortic valve replacement for aortic incompetence ( 27 cases ) , aortic stenosis ( 18 cases ) or mixed aortic valve disease ( 26 cases ) .
	manualset3
207920	6	417932	7	NULL	NULL	0	NULL	isolated aortic valve replacement	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Between January 1970 and December 1982 , seventy-one patients in functional Stage IV of the NYHA classification underwent isolated aortic valve replacement for aortic incompetence ( 27 cases ) , aortic stenosis ( 18 cases ) or mixed aortic valve disease ( 26 cases ) .
	manualset3
207921	7	417932	7	NULL	NULL	0	NULL	aortic incompetence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Between January 1970 and December 1982 , seventy-one patients in functional Stage IV of the NYHA classification underwent isolated aortic valve replacement for aortic incompetence ( 27 cases ) , aortic stenosis ( 18 cases ) or mixed aortic valve disease ( 26 cases ) .
	manualset3
207922	8	417932	7	NULL	NULL	0	NULL	27 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Between January 1970 and December 1982 , seventy-one patients in functional Stage IV of the NYHA classification underwent isolated aortic valve replacement for aortic incompetence ( 27 cases ) , aortic stenosis ( 18 cases ) or mixed aortic valve disease ( 26 cases ) .
	manualset3
207923	9	417932	7	NULL	NULL	NULL	NULL	aortic stenosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between January 1970 and December 1982 , seventy-one patients in functional Stage IV of the NYHA classification underwent isolated aortic valve replacement for aortic incompetence ( 27 cases ) , aortic stenosis ( 18 cases ) or mixed aortic valve disease ( 26 cases ) .
	manualset3
207924	10	417932	7	NULL	NULL	0	NULL	18 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Between January 1970 and December 1982 , seventy-one patients in functional Stage IV of the NYHA classification underwent isolated aortic valve replacement for aortic incompetence ( 27 cases ) , aortic stenosis ( 18 cases ) or mixed aortic valve disease ( 26 cases ) .
	manualset3
207925	11	417932	7	NULL	NULL	0	NULL	mixed aortic valve disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Between January 1970 and December 1982 , seventy-one patients in functional Stage IV of the NYHA classification underwent isolated aortic valve replacement for aortic incompetence ( 27 cases ) , aortic stenosis ( 18 cases ) or mixed aortic valve disease ( 26 cases ) .
	manualset3
207926	12	417932	7	NULL	NULL	0	NULL	26 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Between January 1970 and December 1982 , seventy-one patients in functional Stage IV of the NYHA classification underwent isolated aortic valve replacement for aortic incompetence ( 27 cases ) , aortic stenosis ( 18 cases ) or mixed aortic valve disease ( 26 cases ) .
	manualset3
207927	1	417933	7	NULL	NULL	0	NULL	Patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing oral surgery for impacted mandibular molars should be informed of the anatomical relationship of the lingual nerve to the roots , and the implications of denervation .
	manualset3
207928	2	417933	7	NULL	NULL	0	NULL	oral surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing oral surgery for impacted mandibular molars should be informed of the anatomical relationship of the lingual nerve to the roots , and the implications of denervation .
	manualset3
207929	3	417933	7	NULL	NULL	0	NULL	 impacted mandibular molars	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing oral surgery for impacted mandibular molars should be informed of the anatomical relationship of the lingual nerve to the roots , and the implications of denervation .
	manualset3
207930	4	417933	7	NULL	NULL	0	NULL	anatomical relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing oral surgery for impacted mandibular molars should be informed of the anatomical relationship of the lingual nerve to the roots , and the implications of denervation .
	manualset3
207931	5	417933	7	NULL	NULL	0	NULL	lingual nerve	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing oral surgery for impacted mandibular molars should be informed of the anatomical relationship of the lingual nerve to the roots , and the implications of denervation .
	manualset3
207932	6	417933	7	NULL	NULL	0	NULL	roots	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing oral surgery for impacted mandibular molars should be informed of the anatomical relationship of the lingual nerve to the roots , and the implications of denervation .
	manualset3
207933	7	417933	7	NULL	NULL	0	NULL	implications 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing oral surgery for impacted mandibular molars should be informed of the anatomical relationship of the lingual nerve to the roots , and the implications of denervation .
	manualset3
207934	8	417933	7	NULL	NULL	0	NULL	denervation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients undergoing oral surgery for impacted mandibular molars should be informed of the anatomical relationship of the lingual nerve to the roots , and the implications of denervation .
	manualset3
207935	1	417934	7	NULL	NULL	NULL	NULL	neural network approach	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A neural network approach to a Bayesian statistical decision problem .
	manualset3
207936	2	417934	7	NULL	NULL	0	NULL	Bayesian statistical decision problem	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A neural network approach to a Bayesian statistical decision problem .
	manualset3
207937	1	417935	7	NULL	NULL	0	NULL	Proton NMR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton NMR of lyophilized aortic fragments revealed several peaks originating from biologically relevant molecules , lactate , creatine , taurine ... These preliminary data demonstrate the feasability of multinuclear NMR spectroscopy of vascular tissue and are suggestive of the potential of the method when it will be combined with monitoring of functional parameters .
	manualset3
207938	2	417935	7	NULL	NULL	0	NULL	lyophilized aortic fragments	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton NMR of lyophilized aortic fragments revealed several peaks originating from biologically relevant molecules , lactate , creatine , taurine ... These preliminary data demonstrate the feasability of multinuclear NMR spectroscopy of vascular tissue and are suggestive of the potential of the method when it will be combined with monitoring of functional parameters .
	manualset3
207939	3	417935	7	NULL	NULL	0	NULL	several peaks	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton NMR of lyophilized aortic fragments revealed several peaks originating from biologically relevant molecules , lactate , creatine , taurine ... These preliminary data demonstrate the feasability of multinuclear NMR spectroscopy of vascular tissue and are suggestive of the potential of the method when it will be combined with monitoring of functional parameters .
	manualset3
207940	4	417935	7	NULL	NULL	0	NULL	biologically relevant molecules	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton NMR of lyophilized aortic fragments revealed several peaks originating from biologically relevant molecules , lactate , creatine , taurine ... These preliminary data demonstrate the feasability of multinuclear NMR spectroscopy of vascular tissue and are suggestive of the potential of the method when it will be combined with monitoring of functional parameters .
	manualset3
207941	5	417935	7	NULL	NULL	0	NULL	lactate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton NMR of lyophilized aortic fragments revealed several peaks originating from biologically relevant molecules , lactate , creatine , taurine ... These preliminary data demonstrate the feasability of multinuclear NMR spectroscopy of vascular tissue and are suggestive of the potential of the method when it will be combined with monitoring of functional parameters .
	manualset3
207942	6	417935	7	NULL	NULL	0	NULL	creatine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton NMR of lyophilized aortic fragments revealed several peaks originating from biologically relevant molecules , lactate , creatine , taurine ... These preliminary data demonstrate the feasability of multinuclear NMR spectroscopy of vascular tissue and are suggestive of the potential of the method when it will be combined with monitoring of functional parameters .
	manualset3
207943	7	417935	7	NULL	NULL	0	NULL	 taurine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton NMR of lyophilized aortic fragments revealed several peaks originating from biologically relevant molecules , lactate , creatine , taurine ... These preliminary data demonstrate the feasability of multinuclear NMR spectroscopy of vascular tissue and are suggestive of the potential of the method when it will be combined with monitoring of functional parameters .
	manualset3
207944	8	417935	7	NULL	NULL	0	NULL	 preliminary data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton NMR of lyophilized aortic fragments revealed several peaks originating from biologically relevant molecules , lactate , creatine , taurine ... These preliminary data demonstrate the feasability of multinuclear NMR spectroscopy of vascular tissue and are suggestive of the potential of the method when it will be combined with monitoring of functional parameters .
	manualset3
207945	9	417935	7	NULL	NULL	0	NULL	feasability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton NMR of lyophilized aortic fragments revealed several peaks originating from biologically relevant molecules , lactate , creatine , taurine ... These preliminary data demonstrate the feasability of multinuclear NMR spectroscopy of vascular tissue and are suggestive of the potential of the method when it will be combined with monitoring of functional parameters .
	manualset3
207946	10	417935	7	NULL	NULL	0	NULL	multinuclear NMR spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton NMR of lyophilized aortic fragments revealed several peaks originating from biologically relevant molecules , lactate , creatine , taurine ... These preliminary data demonstrate the feasability of multinuclear NMR spectroscopy of vascular tissue and are suggestive of the potential of the method when it will be combined with monitoring of functional parameters .
	manualset3
207947	11	417935	7	NULL	NULL	0	NULL	vascular tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton NMR of lyophilized aortic fragments revealed several peaks originating from biologically relevant molecules , lactate , creatine , taurine ... These preliminary data demonstrate the feasability of multinuclear NMR spectroscopy of vascular tissue and are suggestive of the potential of the method when it will be combined with monitoring of functional parameters .
	manualset3
207948	12	417935	7	NULL	NULL	0	NULL	 potential	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton NMR of lyophilized aortic fragments revealed several peaks originating from biologically relevant molecules , lactate , creatine , taurine ... These preliminary data demonstrate the feasability of multinuclear NMR spectroscopy of vascular tissue and are suggestive of the potential of the method when it will be combined with monitoring of functional parameters .
	manualset3
207949	13	417935	7	NULL	NULL	0	NULL	method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton NMR of lyophilized aortic fragments revealed several peaks originating from biologically relevant molecules , lactate , creatine , taurine ... These preliminary data demonstrate the feasability of multinuclear NMR spectroscopy of vascular tissue and are suggestive of the potential of the method when it will be combined with monitoring of functional parameters .
	manualset3
207950	14	417935	7	NULL	NULL	0	NULL	 monitoring	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton NMR of lyophilized aortic fragments revealed several peaks originating from biologically relevant molecules , lactate , creatine , taurine ... These preliminary data demonstrate the feasability of multinuclear NMR spectroscopy of vascular tissue and are suggestive of the potential of the method when it will be combined with monitoring of functional parameters .
	manualset3
207951	15	417935	7	NULL	NULL	0	NULL	functional parameters 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Proton NMR of lyophilized aortic fragments revealed several peaks originating from biologically relevant molecules , lactate , creatine , taurine ... These preliminary data demonstrate the feasability of multinuclear NMR spectroscopy of vascular tissue and are suggestive of the potential of the method when it will be combined with monitoring of functional parameters .
	manualset3
207952	1	417936	7	NULL	NULL	0	NULL	onset	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The onset of tissue damage and increases in vascular permeability in the gastrointestinal tract correlate temporally with the changes in PAF-acether synthesis and have previously been shown to be inhibited by PAF-acether antagonists .
	manualset3
207953	2	417936	7	NULL	NULL	0	NULL	tissue damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The onset of tissue damage and increases in vascular permeability in the gastrointestinal tract correlate temporally with the changes in PAF-acether synthesis and have previously been shown to be inhibited by PAF-acether antagonists .
	manualset3
207954	3	417936	7	NULL	NULL	0	NULL	 vascular permeability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The onset of tissue damage and increases in vascular permeability in the gastrointestinal tract correlate temporally with the changes in PAF-acether synthesis and have previously been shown to be inhibited by PAF-acether antagonists .
	manualset3
207955	4	417936	7	NULL	NULL	0	NULL	gastrointestinal tract 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The onset of tissue damage and increases in vascular permeability in the gastrointestinal tract correlate temporally with the changes in PAF-acether synthesis and have previously been shown to be inhibited by PAF-acether antagonists .
	manualset3
207956	5	417936	7	NULL	NULL	0	NULL	changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The onset of tissue damage and increases in vascular permeability in the gastrointestinal tract correlate temporally with the changes in PAF-acether synthesis and have previously been shown to be inhibited by PAF-acether antagonists .
	manualset3
207957	6	417936	7	NULL	NULL	0	NULL	PAF-acether synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The onset of tissue damage and increases in vascular permeability in the gastrointestinal tract correlate temporally with the changes in PAF-acether synthesis and have previously been shown to be inhibited by PAF-acether antagonists .
	manualset3
207958	7	417936	7	NULL	NULL	0	NULL	PAF-acether antagonists	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The onset of tissue damage and increases in vascular permeability in the gastrointestinal tract correlate temporally with the changes in PAF-acether synthesis and have previously been shown to be inhibited by PAF-acether antagonists .
	manualset3
207959	1	417937	7	NULL	NULL	0	NULL	legumes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In legumes , it is not known to which extent vernalization requirement or photoperiod responsiveness are necessary for the development of frost tolerance .
	manualset3
207960	2	417937	7	NULL	NULL	0	NULL	vernalization requirement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In legumes , it is not known to which extent vernalization requirement or photoperiod responsiveness are necessary for the development of frost tolerance .
	manualset3
207961	3	417937	7	NULL	NULL	0	NULL	photoperiod responsiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In legumes , it is not known to which extent vernalization requirement or photoperiod responsiveness are necessary for the development of frost tolerance .
	manualset3
207962	4	417937	7	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In legumes , it is not known to which extent vernalization requirement or photoperiod responsiveness are necessary for the development of frost tolerance .
	manualset3
207963	5	417937	7	NULL	NULL	0	NULL	frost tolerance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In legumes , it is not known to which extent vernalization requirement or photoperiod responsiveness are necessary for the development of frost tolerance .
	manualset3
207964	1	417938	7	NULL	NULL	0	NULL	account 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An account is first given of peculiarities of the proximal femur in childhood .
	manualset3
207965	2	417938	7	NULL	NULL	0	NULL	peculiarities	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An account is first given of peculiarities of the proximal femur in childhood .
	manualset3
207966	3	417938	7	NULL	NULL	0	NULL	proximal femur	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An account is first given of peculiarities of the proximal femur in childhood .
	manualset3
207967	4	417938	7	NULL	NULL	0	NULL	childhood	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An account is first given of peculiarities of the proximal femur in childhood .
	manualset3
207968	1	417939	7	NULL	NULL	0	NULL	increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All these provided the considerable increase of the spring wheat harvest -- by 30.1 % as compared to the control .
	manualset3
207969	2	417939	7	NULL	NULL	0	NULL	spring wheat harvest	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	All these provided the considerable increase of the spring wheat harvest -- by 30.1 % as compared to the control .
	manualset3
207970	3	417939	7	NULL	NULL	0	NULL	30.1 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All these provided the considerable increase of the spring wheat harvest -- by 30.1 % as compared to the control .
	manualset3
207971	4	417939	7	NULL	NULL	0	NULL	 control	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	All these provided the considerable increase of the spring wheat harvest -- by 30.1 % as compared to the control .
	manualset3
207972	1	417940	7	NULL	NULL	0	NULL	Thiopentone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Thiopentone and minaxolone caused intense activity in the duodenum and jejunum ( phase I and phase II of the interdigestive cycle ) , but not the stomach or ileum .
	manualset3
207973	2	417940	7	NULL	NULL	0	NULL	minaxolone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Thiopentone and minaxolone caused intense activity in the duodenum and jejunum ( phase I and phase II of the interdigestive cycle ) , but not the stomach or ileum .
	manualset3
207974	3	417940	7	NULL	NULL	0	NULL	 intense activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thiopentone and minaxolone caused intense activity in the duodenum and jejunum ( phase I and phase II of the interdigestive cycle ) , but not the stomach or ileum .
	manualset3
207975	4	417940	7	NULL	NULL	0	NULL	duodenum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Thiopentone and minaxolone caused intense activity in the duodenum and jejunum ( phase I and phase II of the interdigestive cycle ) , but not the stomach or ileum .
	manualset3
207976	5	417940	7	NULL	NULL	0	NULL	 jejunum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Thiopentone and minaxolone caused intense activity in the duodenum and jejunum ( phase I and phase II of the interdigestive cycle ) , but not the stomach or ileum .
	manualset3
207977	6	417940	7	NULL	NULL	0	NULL	phase I	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thiopentone and minaxolone caused intense activity in the duodenum and jejunum ( phase I and phase II of the interdigestive cycle ) , but not the stomach or ileum .
	manualset3
207978	7	417940	7	NULL	NULL	0	NULL	 phase II	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thiopentone and minaxolone caused intense activity in the duodenum and jejunum ( phase I and phase II of the interdigestive cycle ) , but not the stomach or ileum .
	manualset3
207979	8	417940	7	NULL	NULL	0	NULL	 interdigestive cycle	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thiopentone and minaxolone caused intense activity in the duodenum and jejunum ( phase I and phase II of the interdigestive cycle ) , but not the stomach or ileum .
	manualset3
207980	9	417940	7	NULL	NULL	0	NULL	stomach	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Thiopentone and minaxolone caused intense activity in the duodenum and jejunum ( phase I and phase II of the interdigestive cycle ) , but not the stomach or ileum .
	manualset3
207981	10	417940	7	NULL	NULL	0	NULL	ileum 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Thiopentone and minaxolone caused intense activity in the duodenum and jejunum ( phase I and phase II of the interdigestive cycle ) , but not the stomach or ileum .
	manualset3
207982	1	417941	7	NULL	NULL	0	NULL	Vibrio cholerae O1	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Vibrio cholerae O1 and O139 in less than five years old children hospitalised for watery diarrhoea in Delhi , 1993 .
	manualset3
207983	2	417941	7	NULL	NULL	0	NULL	Vibrio cholerae O139	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Vibrio cholerae O1 and O139 in less than five years old children hospitalised for watery diarrhoea in Delhi , 1993 .
	manualset3
207984	3	417941	7	NULL	NULL	0	NULL	five years old	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Vibrio cholerae O1 and O139 in less than five years old children hospitalised for watery diarrhoea in Delhi , 1993 .
	manualset3
207985	4	417941	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Vibrio cholerae O1 and O139 in less than five years old children hospitalised for watery diarrhoea in Delhi , 1993 .
	manualset3
207986	5	417941	7	NULL	NULL	0	NULL	watery diarrhoea	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Vibrio cholerae O1 and O139 in less than five years old children hospitalised for watery diarrhoea in Delhi , 1993 .
	manualset3
207987	6	417941	7	NULL	NULL	0	NULL	Delhi	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Vibrio cholerae O1 and O139 in less than five years old children hospitalised for watery diarrhoea in Delhi , 1993 .
	manualset3
207988	7	417941	7	NULL	NULL	0	NULL	1993	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Vibrio cholerae O1 and O139 in less than five years old children hospitalised for watery diarrhoea in Delhi , 1993 .
	manualset3
207989	1	417942	7	NULL	NULL	0	NULL	H genome specific repetitive sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The H genome specific repetitive sequence of Elymus trachycaulus , pEt2 , consists of three units of a 337-339 bp repeat aligned in tandem .
	manualset3
207990	2	417942	7	NULL	NULL	0	NULL	Elymus trachycaulus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The H genome specific repetitive sequence of Elymus trachycaulus , pEt2 , consists of three units of a 337-339 bp repeat aligned in tandem .
	manualset3
207991	3	417942	7	NULL	NULL	0	NULL	pEt2	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The H genome specific repetitive sequence of Elymus trachycaulus , pEt2 , consists of three units of a 337-339 bp repeat aligned in tandem .
	manualset3
207992	4	417942	7	NULL	NULL	0	NULL	three units	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The H genome specific repetitive sequence of Elymus trachycaulus , pEt2 , consists of three units of a 337-339 bp repeat aligned in tandem .
	manualset3
207993	5	417942	7	NULL	NULL	0	NULL	337-339 bp repeat	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The H genome specific repetitive sequence of Elymus trachycaulus , pEt2 , consists of three units of a 337-339 bp repeat aligned in tandem .
	manualset3
207994	1	417943	7	NULL	NULL	0	NULL	employee	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	When the employee is willing to be assisted , the behavior can be modified and the necessary level of adaptation can occur .
	manualset3
207995	2	417943	7	NULL	NULL	0	NULL	behavior	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When the employee is willing to be assisted , the behavior can be modified and the necessary level of adaptation can occur .
	manualset3
207996	3	417943	7	NULL	NULL	NULL	NULL	 level of adaptation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When the employee is willing to be assisted , the behavior can be modified and the necessary level of adaptation can occur .
	manualset3
207998	1	417944	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the whole , the results reveal that HT exerts a promising antioxidant potential in protecting the PBMC against TCDD induced oxidative stress , which might be due to the presence of catechol moiety in its structure .
	manualset3
207999	2	417944	7	NULL	NULL	0	NULL	HT	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the whole , the results reveal that HT exerts a promising antioxidant potential in protecting the PBMC against TCDD induced oxidative stress , which might be due to the presence of catechol moiety in its structure .
	manualset3
208000	3	417944	7	NULL	NULL	0	NULL	 antioxidant 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the whole , the results reveal that HT exerts a promising antioxidant potential in protecting the PBMC against TCDD induced oxidative stress , which might be due to the presence of catechol moiety in its structure .
	manualset3
208001	4	417944	7	NULL	NULL	0	NULL	PBMC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	On the whole , the results reveal that HT exerts a promising antioxidant potential in protecting the PBMC against TCDD induced oxidative stress , which might be due to the presence of catechol moiety in its structure .
	manualset3
208002	5	417944	7	NULL	NULL	0	NULL	TCDD	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the whole , the results reveal that HT exerts a promising antioxidant potential in protecting the PBMC against TCDD induced oxidative stress , which might be due to the presence of catechol moiety in its structure .
	manualset3
208003	6	417944	7	NULL	NULL	0	NULL	oxidative stress	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the whole , the results reveal that HT exerts a promising antioxidant potential in protecting the PBMC against TCDD induced oxidative stress , which might be due to the presence of catechol moiety in its structure .
	manualset3
208004	7	417944	7	NULL	NULL	0	NULL	catechol moiety	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the whole , the results reveal that HT exerts a promising antioxidant potential in protecting the PBMC against TCDD induced oxidative stress , which might be due to the presence of catechol moiety in its structure .
	manualset3
208005	8	417944	7	NULL	NULL	0	NULL	 structure 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the whole , the results reveal that HT exerts a promising antioxidant potential in protecting the PBMC against TCDD induced oxidative stress , which might be due to the presence of catechol moiety in its structure .
	manualset3
208006	1	417945	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We thought these results reflected the extent of abnormality in fibrin monomer polymerization .
	manualset3
208007	2	417945	7	NULL	NULL	0	NULL	extent 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We thought these results reflected the extent of abnormality in fibrin monomer polymerization .
	manualset3
208008	3	417945	7	NULL	NULL	0	NULL	abnormality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We thought these results reflected the extent of abnormality in fibrin monomer polymerization .
	manualset3
208009	4	417945	7	NULL	NULL	0	NULL	fibrin monomer polymerization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We thought these results reflected the extent of abnormality in fibrin monomer polymerization .
	manualset3
208010	1	417946	7	NULL	NULL	0	NULL	Mobile pulmonary valve thrombus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mobile pulmonary valve thrombus as a cause of chronic thromboembolic pulmonary hypertension .
	manualset3
208011	2	417946	7	NULL	NULL	NULL	NULL	cause	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mobile pulmonary valve thrombus as a cause of chronic thromboembolic pulmonary hypertension .
	manualset3
208012	3	417946	7	NULL	NULL	0	NULL	chronic thromboembolic pulmonary hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mobile pulmonary valve thrombus as a cause of chronic thromboembolic pulmonary hypertension .
	manualset3
208013	1	417947	7	NULL	NULL	0	NULL	W/W39 genotypes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	All W/W39 genotypes resulted in black-eyed-white anemics with reduced gametogenic activity .
	manualset3
208014	2	417947	7	NULL	NULL	0	NULL	black-eyed-white anemics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All W/W39 genotypes resulted in black-eyed-white anemics with reduced gametogenic activity .
	manualset3
208015	3	417947	7	NULL	NULL	0	NULL	reduced gametogenic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All W/W39 genotypes resulted in black-eyed-white anemics with reduced gametogenic activity .
	manualset3
208016	1	417948	7	NULL	NULL	0	NULL	mammalian cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In mammalian cells , sequences with a high AU content and multiple AUUUA motifs have been shown to cause mRNA instability when present in the 3 ' untranslated regions of several transcripts .
	manualset3
208017	2	417948	7	NULL	NULL	0	NULL	high AU content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In mammalian cells , sequences with a high AU content and multiple AUUUA motifs have been shown to cause mRNA instability when present in the 3 ' untranslated regions of several transcripts .
	manualset3
208018	3	417948	7	NULL	NULL	0	NULL	 multiple AUUUA motifs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In mammalian cells , sequences with a high AU content and multiple AUUUA motifs have been shown to cause mRNA instability when present in the 3 ' untranslated regions of several transcripts .
	manualset3
208019	4	417948	7	NULL	NULL	0	NULL	mRNA instability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In mammalian cells , sequences with a high AU content and multiple AUUUA motifs have been shown to cause mRNA instability when present in the 3 ' untranslated regions of several transcripts .
	manualset3
208020	5	417948	7	NULL	NULL	0	NULL	3 ' untranslated regions	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In mammalian cells , sequences with a high AU content and multiple AUUUA motifs have been shown to cause mRNA instability when present in the 3 ' untranslated regions of several transcripts .
	manualset3
208021	6	417948	7	NULL	NULL	0	NULL	transcripts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In mammalian cells , sequences with a high AU content and multiple AUUUA motifs have been shown to cause mRNA instability when present in the 3 ' untranslated regions of several transcripts .
	manualset3
208022	1	417949	7	NULL	NULL	0	NULL	imbalance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An imbalance of Hcy in the body may lead to hyperhomocysteinemia , a condition with elevated Hcy concentration in blood that may be one of the risk factors responsible for the development of several vascular diseases ( thromboembolism , atherosclerosis , stroke , vascular diseases and dementia ) .
	manualset3
208023	2	417949	7	NULL	NULL	0	NULL	Hcy	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An imbalance of Hcy in the body may lead to hyperhomocysteinemia , a condition with elevated Hcy concentration in blood that may be one of the risk factors responsible for the development of several vascular diseases ( thromboembolism , atherosclerosis , stroke , vascular diseases and dementia ) .
	manualset3
208024	3	417949	7	NULL	NULL	0	NULL	body	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An imbalance of Hcy in the body may lead to hyperhomocysteinemia , a condition with elevated Hcy concentration in blood that may be one of the risk factors responsible for the development of several vascular diseases ( thromboembolism , atherosclerosis , stroke , vascular diseases and dementia ) .
	manualset3
208025	4	417949	7	NULL	NULL	NULL	NULL	hyperhomocysteinemia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An imbalance of Hcy in the body may lead to hyperhomocysteinemia , a condition with elevated Hcy concentration in blood that may be one of the risk factors responsible for the development of several vascular diseases ( thromboembolism , atherosclerosis , stroke , vascular diseases and dementia ) .
	manualset3
208026	5	417949	7	NULL	NULL	0	NULL	condition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An imbalance of Hcy in the body may lead to hyperhomocysteinemia , a condition with elevated Hcy concentration in blood that may be one of the risk factors responsible for the development of several vascular diseases ( thromboembolism , atherosclerosis , stroke , vascular diseases and dementia ) .
	manualset3
208027	6	417949	7	NULL	NULL	0	NULL	elevated Hcy concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An imbalance of Hcy in the body may lead to hyperhomocysteinemia , a condition with elevated Hcy concentration in blood that may be one of the risk factors responsible for the development of several vascular diseases ( thromboembolism , atherosclerosis , stroke , vascular diseases and dementia ) .
	manualset3
208028	7	417949	7	NULL	NULL	0	NULL	blood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An imbalance of Hcy in the body may lead to hyperhomocysteinemia , a condition with elevated Hcy concentration in blood that may be one of the risk factors responsible for the development of several vascular diseases ( thromboembolism , atherosclerosis , stroke , vascular diseases and dementia ) .
	manualset3
208029	8	417949	7	NULL	NULL	0	NULL	 risk factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An imbalance of Hcy in the body may lead to hyperhomocysteinemia , a condition with elevated Hcy concentration in blood that may be one of the risk factors responsible for the development of several vascular diseases ( thromboembolism , atherosclerosis , stroke , vascular diseases and dementia ) .
	manualset3
208030	9	417949	7	NULL	NULL	0	NULL	development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An imbalance of Hcy in the body may lead to hyperhomocysteinemia , a condition with elevated Hcy concentration in blood that may be one of the risk factors responsible for the development of several vascular diseases ( thromboembolism , atherosclerosis , stroke , vascular diseases and dementia ) .
	manualset3
208031	10	417949	7	NULL	NULL	0	NULL	several vascular diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	An imbalance of Hcy in the body may lead to hyperhomocysteinemia , a condition with elevated Hcy concentration in blood that may be one of the risk factors responsible for the development of several vascular diseases ( thromboembolism , atherosclerosis , stroke , vascular diseases and dementia ) .
	manualset3
208032	11	417949	7	NULL	NULL	0	NULL	thromboembolism	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	An imbalance of Hcy in the body may lead to hyperhomocysteinemia , a condition with elevated Hcy concentration in blood that may be one of the risk factors responsible for the development of several vascular diseases ( thromboembolism , atherosclerosis , stroke , vascular diseases and dementia ) .
	manualset3
208033	12	417949	7	NULL	NULL	0	NULL	atherosclerosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	An imbalance of Hcy in the body may lead to hyperhomocysteinemia , a condition with elevated Hcy concentration in blood that may be one of the risk factors responsible for the development of several vascular diseases ( thromboembolism , atherosclerosis , stroke , vascular diseases and dementia ) .
	manualset3
208034	13	417949	7	NULL	NULL	0	NULL	stroke	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	An imbalance of Hcy in the body may lead to hyperhomocysteinemia , a condition with elevated Hcy concentration in blood that may be one of the risk factors responsible for the development of several vascular diseases ( thromboembolism , atherosclerosis , stroke , vascular diseases and dementia ) .
	manualset3
208035	14	417949	7	NULL	NULL	0	NULL	vascular diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	An imbalance of Hcy in the body may lead to hyperhomocysteinemia , a condition with elevated Hcy concentration in blood that may be one of the risk factors responsible for the development of several vascular diseases ( thromboembolism , atherosclerosis , stroke , vascular diseases and dementia ) .
	manualset3
208036	15	417949	7	NULL	NULL	0	NULL	dementia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	An imbalance of Hcy in the body may lead to hyperhomocysteinemia , a condition with elevated Hcy concentration in blood that may be one of the risk factors responsible for the development of several vascular diseases ( thromboembolism , atherosclerosis , stroke , vascular diseases and dementia ) .
	manualset3
208037	1	417950	7	NULL	NULL	0	NULL	 subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The subjects were requested to respond to verbal tasks ( counting , picture description , story telling ) .
	manualset3
208038	2	417950	7	NULL	NULL	0	NULL	verbal tasks	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The subjects were requested to respond to verbal tasks ( counting , picture description , story telling ) .
	manualset3
208039	3	417950	7	NULL	NULL	0	NULL	counting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The subjects were requested to respond to verbal tasks ( counting , picture description , story telling ) .
	manualset3
208040	4	417950	7	NULL	NULL	0	NULL	picture description	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The subjects were requested to respond to verbal tasks ( counting , picture description , story telling ) .
	manualset3
208041	5	417950	7	NULL	NULL	0	NULL	 story telling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The subjects were requested to respond to verbal tasks ( counting , picture description , story telling ) .
	manualset3
208042	1	417951	7	NULL	NULL	0	NULL	2 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For 2 mM sodium saccharin ( NaSac ) , 75 % of the responses were `` sweet , '' 6.5 % `` sugar '' ; for NaSac in 10 mM citric acid ( ArtLem ) , 43 % `` sour , '' 20 % `` citrus , '' and 11 % `` sugar '' ; for 214 mM monosodium glutamate ( MSG ) , 28 % `` salty , '' 14 % `` sour , '' and 10 % 1st `` soapy , '' then `` no taste , '' and finally `` bitter . ''
	manualset3
208043	2	417951	7	NULL	NULL	0	NULL	sodium saccharin ( NaSac )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For 2 mM sodium saccharin ( NaSac ) , 75 % of the responses were `` sweet , '' 6.5 % `` sugar '' ; for NaSac in 10 mM citric acid ( ArtLem ) , 43 % `` sour , '' 20 % `` citrus , '' and 11 % `` sugar '' ; for 214 mM monosodium glutamate ( MSG ) , 28 % `` salty , '' 14 % `` sour , '' and 10 % 1st `` soapy , '' then `` no taste , '' and finally `` bitter . ''
	manualset3
208044	3	417951	7	NULL	NULL	0	NULL	75 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For 2 mM sodium saccharin ( NaSac ) , 75 % of the responses were `` sweet , '' 6.5 % `` sugar '' ; for NaSac in 10 mM citric acid ( ArtLem ) , 43 % `` sour , '' 20 % `` citrus , '' and 11 % `` sugar '' ; for 214 mM monosodium glutamate ( MSG ) , 28 % `` salty , '' 14 % `` sour , '' and 10 % 1st `` soapy , '' then `` no taste , '' and finally `` bitter . ''
	manualset3
208045	4	417951	7	NULL	NULL	NULL	NULL	responses	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For 2 mM sodium saccharin ( NaSac ) , 75 % of the responses were `` sweet , '' 6.5 % `` sugar '' ; for NaSac in 10 mM citric acid ( ArtLem ) , 43 % `` sour , '' 20 % `` citrus , '' and 11 % `` sugar '' ; for 214 mM monosodium glutamate ( MSG ) , 28 % `` salty , '' 14 % `` sour , '' and 10 % 1st `` soapy , '' then `` no taste , '' and finally `` bitter . ''
	manualset3
208047	6	417951	7	NULL	NULL	0	NULL	6.5 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For 2 mM sodium saccharin ( NaSac ) , 75 % of the responses were `` sweet , '' 6.5 % `` sugar '' ; for NaSac in 10 mM citric acid ( ArtLem ) , 43 % `` sour , '' 20 % `` citrus , '' and 11 % `` sugar '' ; for 214 mM monosodium glutamate ( MSG ) , 28 % `` salty , '' 14 % `` sour , '' and 10 % 1st `` soapy , '' then `` no taste , '' and finally `` bitter . ''
	manualset3
208048	7	417951	7	NULL	NULL	0	NULL	sugar	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	For 2 mM sodium saccharin ( NaSac ) , 75 % of the responses were `` sweet , '' 6.5 % `` sugar '' ; for NaSac in 10 mM citric acid ( ArtLem ) , 43 % `` sour , '' 20 % `` citrus , '' and 11 % `` sugar '' ; for 214 mM monosodium glutamate ( MSG ) , 28 % `` salty , '' 14 % `` sour , '' and 10 % 1st `` soapy , '' then `` no taste , '' and finally `` bitter . ''
	manualset3
208049	8	417951	7	NULL	NULL	0	NULL	NaSac	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For 2 mM sodium saccharin ( NaSac ) , 75 % of the responses were `` sweet , '' 6.5 % `` sugar '' ; for NaSac in 10 mM citric acid ( ArtLem ) , 43 % `` sour , '' 20 % `` citrus , '' and 11 % `` sugar '' ; for 214 mM monosodium glutamate ( MSG ) , 28 % `` salty , '' 14 % `` sour , '' and 10 % 1st `` soapy , '' then `` no taste , '' and finally `` bitter . ''
	manualset3
208050	9	417951	7	NULL	NULL	0	NULL	10 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For 2 mM sodium saccharin ( NaSac ) , 75 % of the responses were `` sweet , '' 6.5 % `` sugar '' ; for NaSac in 10 mM citric acid ( ArtLem ) , 43 % `` sour , '' 20 % `` citrus , '' and 11 % `` sugar '' ; for 214 mM monosodium glutamate ( MSG ) , 28 % `` salty , '' 14 % `` sour , '' and 10 % 1st `` soapy , '' then `` no taste , '' and finally `` bitter . ''
	manualset3
208051	10	417951	7	NULL	NULL	0	NULL	citric acid ( ArtLem )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For 2 mM sodium saccharin ( NaSac ) , 75 % of the responses were `` sweet , '' 6.5 % `` sugar '' ; for NaSac in 10 mM citric acid ( ArtLem ) , 43 % `` sour , '' 20 % `` citrus , '' and 11 % `` sugar '' ; for 214 mM monosodium glutamate ( MSG ) , 28 % `` salty , '' 14 % `` sour , '' and 10 % 1st `` soapy , '' then `` no taste , '' and finally `` bitter . ''
	manualset3
208052	11	417951	7	NULL	NULL	0	NULL	43 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For 2 mM sodium saccharin ( NaSac ) , 75 % of the responses were `` sweet , '' 6.5 % `` sugar '' ; for NaSac in 10 mM citric acid ( ArtLem ) , 43 % `` sour , '' 20 % `` citrus , '' and 11 % `` sugar '' ; for 214 mM monosodium glutamate ( MSG ) , 28 % `` salty , '' 14 % `` sour , '' and 10 % 1st `` soapy , '' then `` no taste , '' and finally `` bitter . ''
	manualset3
208054	13	417951	7	NULL	NULL	0	NULL	20 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For 2 mM sodium saccharin ( NaSac ) , 75 % of the responses were `` sweet , '' 6.5 % `` sugar '' ; for NaSac in 10 mM citric acid ( ArtLem ) , 43 % `` sour , '' 20 % `` citrus , '' and 11 % `` sugar '' ; for 214 mM monosodium glutamate ( MSG ) , 28 % `` salty , '' 14 % `` sour , '' and 10 % 1st `` soapy , '' then `` no taste , '' and finally `` bitter . ''
	manualset3
208055	14	417951	7	NULL	NULL	0	NULL	 citrus	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	For 2 mM sodium saccharin ( NaSac ) , 75 % of the responses were `` sweet , '' 6.5 % `` sugar '' ; for NaSac in 10 mM citric acid ( ArtLem ) , 43 % `` sour , '' 20 % `` citrus , '' and 11 % `` sugar '' ; for 214 mM monosodium glutamate ( MSG ) , 28 % `` salty , '' 14 % `` sour , '' and 10 % 1st `` soapy , '' then `` no taste , '' and finally `` bitter . ''
	manualset3
208056	15	417951	7	NULL	NULL	0	NULL	11 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For 2 mM sodium saccharin ( NaSac ) , 75 % of the responses were `` sweet , '' 6.5 % `` sugar '' ; for NaSac in 10 mM citric acid ( ArtLem ) , 43 % `` sour , '' 20 % `` citrus , '' and 11 % `` sugar '' ; for 214 mM monosodium glutamate ( MSG ) , 28 % `` salty , '' 14 % `` sour , '' and 10 % 1st `` soapy , '' then `` no taste , '' and finally `` bitter . ''
	manualset3
208057	16	417951	7	NULL	NULL	0	NULL	sugar 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	For 2 mM sodium saccharin ( NaSac ) , 75 % of the responses were `` sweet , '' 6.5 % `` sugar '' ; for NaSac in 10 mM citric acid ( ArtLem ) , 43 % `` sour , '' 20 % `` citrus , '' and 11 % `` sugar '' ; for 214 mM monosodium glutamate ( MSG ) , 28 % `` salty , '' 14 % `` sour , '' and 10 % 1st `` soapy , '' then `` no taste , '' and finally `` bitter . ''
	manualset3
208058	17	417951	7	NULL	NULL	0	NULL	214 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For 2 mM sodium saccharin ( NaSac ) , 75 % of the responses were `` sweet , '' 6.5 % `` sugar '' ; for NaSac in 10 mM citric acid ( ArtLem ) , 43 % `` sour , '' 20 % `` citrus , '' and 11 % `` sugar '' ; for 214 mM monosodium glutamate ( MSG ) , 28 % `` salty , '' 14 % `` sour , '' and 10 % 1st `` soapy , '' then `` no taste , '' and finally `` bitter . ''
	manualset3
208059	18	417951	7	NULL	NULL	0	NULL	monosodium glutamate ( MSG )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For 2 mM sodium saccharin ( NaSac ) , 75 % of the responses were `` sweet , '' 6.5 % `` sugar '' ; for NaSac in 10 mM citric acid ( ArtLem ) , 43 % `` sour , '' 20 % `` citrus , '' and 11 % `` sugar '' ; for 214 mM monosodium glutamate ( MSG ) , 28 % `` salty , '' 14 % `` sour , '' and 10 % 1st `` soapy , '' then `` no taste , '' and finally `` bitter . ''
	manualset3
208060	19	417951	7	NULL	NULL	0	NULL	28 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For 2 mM sodium saccharin ( NaSac ) , 75 % of the responses were `` sweet , '' 6.5 % `` sugar '' ; for NaSac in 10 mM citric acid ( ArtLem ) , 43 % `` sour , '' 20 % `` citrus , '' and 11 % `` sugar '' ; for 214 mM monosodium glutamate ( MSG ) , 28 % `` salty , '' 14 % `` sour , '' and 10 % 1st `` soapy , '' then `` no taste , '' and finally `` bitter . ''
	manualset3
208062	21	417951	7	NULL	NULL	0	NULL	14 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For 2 mM sodium saccharin ( NaSac ) , 75 % of the responses were `` sweet , '' 6.5 % `` sugar '' ; for NaSac in 10 mM citric acid ( ArtLem ) , 43 % `` sour , '' 20 % `` citrus , '' and 11 % `` sugar '' ; for 214 mM monosodium glutamate ( MSG ) , 28 % `` salty , '' 14 % `` sour , '' and 10 % 1st `` soapy , '' then `` no taste , '' and finally `` bitter . ''
	manualset3
208064	23	417951	7	NULL	NULL	0	NULL	10 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For 2 mM sodium saccharin ( NaSac ) , 75 % of the responses were `` sweet , '' 6.5 % `` sugar '' ; for NaSac in 10 mM citric acid ( ArtLem ) , 43 % `` sour , '' 20 % `` citrus , '' and 11 % `` sugar '' ; for 214 mM monosodium glutamate ( MSG ) , 28 % `` salty , '' 14 % `` sour , '' and 10 % 1st `` soapy , '' then `` no taste , '' and finally `` bitter . ''
	manualset3
208066	25	417951	7	NULL	NULL	NULL	NULL	 no taste	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For 2 mM sodium saccharin ( NaSac ) , 75 % of the responses were `` sweet , '' 6.5 % `` sugar '' ; for NaSac in 10 mM citric acid ( ArtLem ) , 43 % `` sour , '' 20 % `` citrus , '' and 11 % `` sugar '' ; for 214 mM monosodium glutamate ( MSG ) , 28 % `` salty , '' 14 % `` sour , '' and 10 % 1st `` soapy , '' then `` no taste , '' and finally `` bitter . ''
	manualset3
208068	1	417952	7	NULL	NULL	0	NULL	reverse genetics approach 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Utilizing a reverse genetics approach , we have isolated the cDNAs encoding two distinct fiber coating products , which we have named spider coating peptide 1 and 2 ( SCP-1 and SCP-2 ) .
	manualset3
208069	2	417952	7	NULL	NULL	0	NULL	cDNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Utilizing a reverse genetics approach , we have isolated the cDNAs encoding two distinct fiber coating products , which we have named spider coating peptide 1 and 2 ( SCP-1 and SCP-2 ) .
	manualset3
208070	3	417952	7	NULL	NULL	NULL	NULL	 two distinct fiber coating products	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Utilizing a reverse genetics approach , we have isolated the cDNAs encoding two distinct fiber coating products , which we have named spider coating peptide 1 and 2 ( SCP-1 and SCP-2 ) .
	manualset3
208071	4	417952	7	NULL	NULL	0	NULL	spider coating peptide 1	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Utilizing a reverse genetics approach , we have isolated the cDNAs encoding two distinct fiber coating products , which we have named spider coating peptide 1 and 2 ( SCP-1 and SCP-2 ) .
	manualset3
208072	5	417952	7	NULL	NULL	0	NULL	spider coating peptide 2	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Utilizing a reverse genetics approach , we have isolated the cDNAs encoding two distinct fiber coating products , which we have named spider coating peptide 1 and 2 ( SCP-1 and SCP-2 ) .
	manualset3
208073	6	417952	7	NULL	NULL	0	NULL	SCP-1 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Utilizing a reverse genetics approach , we have isolated the cDNAs encoding two distinct fiber coating products , which we have named spider coating peptide 1 and 2 ( SCP-1 and SCP-2 ) .
	manualset3
208074	7	417952	7	NULL	NULL	0	NULL	SCP-2	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Utilizing a reverse genetics approach , we have isolated the cDNAs encoding two distinct fiber coating products , which we have named spider coating peptide 1 and 2 ( SCP-1 and SCP-2 ) .
	manualset3
208075	1	417953	7	NULL	NULL	0	NULL	Gastrostomy insertion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrostomy insertion in the 21st century : PEG or laparoscopic ?
	manualset3
208076	2	417953	7	NULL	NULL	0	NULL	21st century	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrostomy insertion in the 21st century : PEG or laparoscopic ?
	manualset3
208077	3	417953	7	NULL	NULL	0	NULL	PEG	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrostomy insertion in the 21st century : PEG or laparoscopic ?
	manualset3
208078	4	417953	7	NULL	NULL	0	NULL	 laparoscopic	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrostomy insertion in the 21st century : PEG or laparoscopic ?
	manualset3
208079	1	417954	7	NULL	NULL	0	NULL	cardiac hypertrophy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Because cardiac hypertrophy can progress to heart failure , a major cause of lethality worldwide , the intracellular signaling pathways that control cardiomyocyte growth have been the subject of intensive investigation .
	manualset3
208080	2	417954	7	NULL	NULL	0	NULL	 heart failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Because cardiac hypertrophy can progress to heart failure , a major cause of lethality worldwide , the intracellular signaling pathways that control cardiomyocyte growth have been the subject of intensive investigation .
	manualset3
208081	3	417954	7	NULL	NULL	0	NULL	major cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Because cardiac hypertrophy can progress to heart failure , a major cause of lethality worldwide , the intracellular signaling pathways that control cardiomyocyte growth have been the subject of intensive investigation .
	manualset3
208082	4	417954	7	NULL	NULL	NULL	NULL	lethality	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because cardiac hypertrophy can progress to heart failure , a major cause of lethality worldwide , the intracellular signaling pathways that control cardiomyocyte growth have been the subject of intensive investigation .
	manualset3
208083	5	417954	7	NULL	NULL	0	NULL	intracellular signaling pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Because cardiac hypertrophy can progress to heart failure , a major cause of lethality worldwide , the intracellular signaling pathways that control cardiomyocyte growth have been the subject of intensive investigation .
	manualset3
208084	6	417954	7	NULL	NULL	0	NULL	cardiomyocyte growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Because cardiac hypertrophy can progress to heart failure , a major cause of lethality worldwide , the intracellular signaling pathways that control cardiomyocyte growth have been the subject of intensive investigation .
	manualset3
208085	7	417954	7	NULL	NULL	0	NULL	subject 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Because cardiac hypertrophy can progress to heart failure , a major cause of lethality worldwide , the intracellular signaling pathways that control cardiomyocyte growth have been the subject of intensive investigation .
	manualset3
208086	8	417954	7	NULL	NULL	0	NULL	intensive investigation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Because cardiac hypertrophy can progress to heart failure , a major cause of lethality worldwide , the intracellular signaling pathways that control cardiomyocyte growth have been the subject of intensive investigation .
	manualset3
208087	1	417955	7	NULL	NULL	0	NULL	 Cuban PCV2 sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	All the Cuban PCV2 sequences analyzed belonged to genotype 1 and were located within the same Cluster ( 1A ) .
	manualset3
208088	2	417955	7	NULL	NULL	0	NULL	genotype 1 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	All the Cuban PCV2 sequences analyzed belonged to genotype 1 and were located within the same Cluster ( 1A ) .
	manualset3
208089	3	417955	7	NULL	NULL	0	NULL	 Cluster ( 1A )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	All the Cuban PCV2 sequences analyzed belonged to genotype 1 and were located within the same Cluster ( 1A ) .
	manualset3
208090	1	417956	7	NULL	NULL	0	NULL	Staining	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Staining of life sperm cells indicated that the antigen is present on the sperm surface .
	manualset3
208091	2	417956	7	NULL	NULL	0	NULL	life sperm cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Staining of life sperm cells indicated that the antigen is present on the sperm surface .
	manualset3
208092	3	417956	7	NULL	NULL	0	NULL	antigen	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Staining of life sperm cells indicated that the antigen is present on the sperm surface .
	manualset3
208093	4	417956	7	NULL	NULL	0	NULL	sperm surface	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Staining of life sperm cells indicated that the antigen is present on the sperm surface .
	manualset3
208094	1	417957	7	NULL	NULL	0	NULL	site of damage	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The site of damage in the kidney tubule is consistent with the region of concentration of filtered FeNTA .
	manualset3
208095	2	417957	7	NULL	NULL	0	NULL	kidney tubule	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The site of damage in the kidney tubule is consistent with the region of concentration of filtered FeNTA .
	manualset3
208096	3	417957	7	NULL	NULL	0	NULL	region of concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The site of damage in the kidney tubule is consistent with the region of concentration of filtered FeNTA .
	manualset3
208097	4	417957	7	NULL	NULL	0	NULL	filtered FeNTA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The site of damage in the kidney tubule is consistent with the region of concentration of filtered FeNTA .
	manualset3
208098	1	417958	7	NULL	NULL	0	NULL	PC1	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In PC1 , pH was lower than 6.3 , and platelet function and discoid morphology were lost .
	manualset3
208099	2	417958	7	NULL	NULL	0	NULL	pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In PC1 , pH was lower than 6.3 , and platelet function and discoid morphology were lost .
	manualset3
208100	3	417958	7	NULL	NULL	0	NULL	6.3	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In PC1 , pH was lower than 6.3 , and platelet function and discoid morphology were lost .
	manualset3
208101	4	417958	7	NULL	NULL	0	NULL	platelet function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In PC1 , pH was lower than 6.3 , and platelet function and discoid morphology were lost .
	manualset3
208102	5	417958	7	NULL	NULL	NULL	NULL	discoid morphology	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In PC1 , pH was lower than 6.3 , and platelet function and discoid morphology were lost .
	manualset3
208103	1	417959	7	NULL	NULL	0	NULL	 alpha-tocopherol / ( cholesterol + triglycerides ) ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also related to the alpha-tocopherol / ( cholesterol + triglycerides ) ratio in plasma ( r = .431 ; P & lt ; .04 ) .
	manualset3
208104	2	417959	7	NULL	NULL	0	NULL	plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also related to the alpha-tocopherol / ( cholesterol + triglycerides ) ratio in plasma ( r = .431 ; P & lt ; .04 ) .
	manualset3
208105	3	417959	7	NULL	NULL	0	NULL	r = .431	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also related to the alpha-tocopherol / ( cholesterol + triglycerides ) ratio in plasma ( r = .431 ; P & lt ; .04 ) .
	manualset3
208106	4	417959	7	NULL	NULL	0	NULL	P & lt ; .04	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also related to the alpha-tocopherol / ( cholesterol + triglycerides ) ratio in plasma ( r = .431 ; P & lt ; .04 ) .
	manualset3
208107	1	417960	7	NULL	NULL	0	NULL	Rabbits	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rabbits that have been exposed to the natural cycles of day and night exhibit marked diurnal changes in the shape of their Visual Evoked Potential in constant environmental conditions .
	manualset3
208108	2	417960	7	NULL	NULL	0	NULL	natural cycles	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rabbits that have been exposed to the natural cycles of day and night exhibit marked diurnal changes in the shape of their Visual Evoked Potential in constant environmental conditions .
	manualset3
208109	3	417960	7	NULL	NULL	0	NULL	day 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Rabbits that have been exposed to the natural cycles of day and night exhibit marked diurnal changes in the shape of their Visual Evoked Potential in constant environmental conditions .
	manualset3
208110	4	417960	7	NULL	NULL	0	NULL	night	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Rabbits that have been exposed to the natural cycles of day and night exhibit marked diurnal changes in the shape of their Visual Evoked Potential in constant environmental conditions .
	manualset3
208111	5	417960	7	NULL	NULL	0	NULL	diurnal changes 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rabbits that have been exposed to the natural cycles of day and night exhibit marked diurnal changes in the shape of their Visual Evoked Potential in constant environmental conditions .
	manualset3
208112	6	417960	7	NULL	NULL	0	NULL	shape	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Rabbits that have been exposed to the natural cycles of day and night exhibit marked diurnal changes in the shape of their Visual Evoked Potential in constant environmental conditions .
	manualset3
208113	7	417960	7	NULL	NULL	0	NULL	Visual Evoked Potential	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Rabbits that have been exposed to the natural cycles of day and night exhibit marked diurnal changes in the shape of their Visual Evoked Potential in constant environmental conditions .
	manualset3
208114	8	417960	7	NULL	NULL	0	NULL	constant environmental conditions	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Rabbits that have been exposed to the natural cycles of day and night exhibit marked diurnal changes in the shape of their Visual Evoked Potential in constant environmental conditions .
	manualset3
208115	1	417961	7	NULL	NULL	0	NULL	Innate immunity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Innate , inflammation-based immunity is the first line of vertebrate defense against micro-organisms .
	manualset3
208116	2	417961	7	NULL	NULL	0	NULL	inflammation-based immunity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Innate , inflammation-based immunity is the first line of vertebrate defense against micro-organisms .
	manualset3
208117	3	417961	7	NULL	NULL	0	NULL	first line	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Innate , inflammation-based immunity is the first line of vertebrate defense against micro-organisms .
	manualset3
208118	4	417961	7	NULL	NULL	0	NULL	vertebrate	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Innate , inflammation-based immunity is the first line of vertebrate defense against micro-organisms .
	manualset3
208119	5	417961	7	NULL	NULL	0	NULL	micro-organisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Innate , inflammation-based immunity is the first line of vertebrate defense against micro-organisms .
	manualset3
208120	1	417962	7	NULL	NULL	0	NULL	intrinsic helix stability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that intrinsic helix stability is a major determinant of the folding rate of the GCN4 coiled coil .
	manualset3
208121	2	417962	7	NULL	NULL	0	NULL	determinant	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that intrinsic helix stability is a major determinant of the folding rate of the GCN4 coiled coil .
	manualset3
208122	3	417962	7	NULL	NULL	0	NULL	folding rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that intrinsic helix stability is a major determinant of the folding rate of the GCN4 coiled coil .
	manualset3
208123	4	417962	7	NULL	NULL	0	NULL	GCN4 coiled coil	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that intrinsic helix stability is a major determinant of the folding rate of the GCN4 coiled coil .
	manualset3
208124	1	417963	7	NULL	NULL	0	NULL	Plasma total catecholamine levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma total catecholamine and specifically plasma-noradrenaline levels were significantly higher in the three hours before the subjects awoke with migraine .
	manualset3
208125	2	417963	7	NULL	NULL	0	NULL	plasma-noradrenaline levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma total catecholamine and specifically plasma-noradrenaline levels were significantly higher in the three hours before the subjects awoke with migraine .
	manualset3
208126	3	417963	7	NULL	NULL	0	NULL	 three hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma total catecholamine and specifically plasma-noradrenaline levels were significantly higher in the three hours before the subjects awoke with migraine .
	manualset3
208127	4	417963	7	NULL	NULL	0	NULL	subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasma total catecholamine and specifically plasma-noradrenaline levels were significantly higher in the three hours before the subjects awoke with migraine .
	manualset3
208128	5	417963	7	NULL	NULL	NULL	NULL	migraine 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Plasma total catecholamine and specifically plasma-noradrenaline levels were significantly higher in the three hours before the subjects awoke with migraine .
	manualset3
208129	1	417964	7	NULL	NULL	0	NULL	RFLP types	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	All the RFLP types and detailed protocols are available at Intemet web site WWW ... : http : / / www.vri.cz/wwwrflptext.htm .
	manualset3
208130	2	417964	7	NULL	NULL	0	NULL	detailed protocols	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	All the RFLP types and detailed protocols are available at Intemet web site WWW ... : http : / / www.vri.cz/wwwrflptext.htm .
	manualset3
208131	3	417964	7	NULL	NULL	0	NULL	Intemet web site	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	All the RFLP types and detailed protocols are available at Intemet web site WWW ... : http : / / www.vri.cz/wwwrflptext.htm .
	manualset3
208132	4	417964	7	NULL	NULL	0	NULL	WWW ... : http : / / www.vri.cz/wwwrflptext.htm 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	All the RFLP types and detailed protocols are available at Intemet web site WWW ... : http : / / www.vri.cz/wwwrflptext.htm .
	manualset3
208133	1	417965	7	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of cement produced a significant reduction in migration at one year , from a mean of 1.5 mm to one of 0.5 mm ( p less than 0.01 ) , including a significant reduction in pure subsidence .
	manualset3
208134	2	417965	7	NULL	NULL	0	NULL	cement	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of cement produced a significant reduction in migration at one year , from a mean of 1.5 mm to one of 0.5 mm ( p less than 0.01 ) , including a significant reduction in pure subsidence .
	manualset3
208135	3	417965	7	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of cement produced a significant reduction in migration at one year , from a mean of 1.5 mm to one of 0.5 mm ( p less than 0.01 ) , including a significant reduction in pure subsidence .
	manualset3
208136	4	417965	7	NULL	NULL	0	NULL	migration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of cement produced a significant reduction in migration at one year , from a mean of 1.5 mm to one of 0.5 mm ( p less than 0.01 ) , including a significant reduction in pure subsidence .
	manualset3
208137	5	417965	7	NULL	NULL	0	NULL	one year	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of cement produced a significant reduction in migration at one year , from a mean of 1.5 mm to one of 0.5 mm ( p less than 0.01 ) , including a significant reduction in pure subsidence .
	manualset3
208138	6	417965	7	NULL	NULL	0	NULL	mean	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of cement produced a significant reduction in migration at one year , from a mean of 1.5 mm to one of 0.5 mm ( p less than 0.01 ) , including a significant reduction in pure subsidence .
	manualset3
208139	7	417965	7	NULL	NULL	0	NULL	1.5 mm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of cement produced a significant reduction in migration at one year , from a mean of 1.5 mm to one of 0.5 mm ( p less than 0.01 ) , including a significant reduction in pure subsidence .
	manualset3
208140	8	417965	7	NULL	NULL	0	NULL	 one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of cement produced a significant reduction in migration at one year , from a mean of 1.5 mm to one of 0.5 mm ( p less than 0.01 ) , including a significant reduction in pure subsidence .
	manualset3
208141	9	417965	7	NULL	NULL	0	NULL	 0.5 mm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of cement produced a significant reduction in migration at one year , from a mean of 1.5 mm to one of 0.5 mm ( p less than 0.01 ) , including a significant reduction in pure subsidence .
	manualset3
208142	10	417965	7	NULL	NULL	0	NULL	p less than 0.01	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of cement produced a significant reduction in migration at one year , from a mean of 1.5 mm to one of 0.5 mm ( p less than 0.01 ) , including a significant reduction in pure subsidence .
	manualset3
208143	11	417965	7	NULL	NULL	0	NULL	 reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of cement produced a significant reduction in migration at one year , from a mean of 1.5 mm to one of 0.5 mm ( p less than 0.01 ) , including a significant reduction in pure subsidence .
	manualset3
208144	12	417965	7	NULL	NULL	0	NULL	pure subsidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of cement produced a significant reduction in migration at one year , from a mean of 1.5 mm to one of 0.5 mm ( p less than 0.01 ) , including a significant reduction in pure subsidence .
	manualset3
208145	1	417966	7	NULL	NULL	0	NULL	Estrogen-related proliferation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Estrogen-related proliferation in ROS17/2 .8 cells appears to be mediated by IGF-I acting through the IGF-I receptor and does not involve IGF-II .
	manualset3
208146	2	417966	7	NULL	NULL	0	NULL	ROS17/2 .8 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Estrogen-related proliferation in ROS17/2 .8 cells appears to be mediated by IGF-I acting through the IGF-I receptor and does not involve IGF-II .
	manualset3
208147	3	417966	7	NULL	NULL	0	NULL	IGF-I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Estrogen-related proliferation in ROS17/2 .8 cells appears to be mediated by IGF-I acting through the IGF-I receptor and does not involve IGF-II .
	manualset3
208148	4	417966	7	NULL	NULL	0	NULL	 IGF-I receptor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Estrogen-related proliferation in ROS17/2 .8 cells appears to be mediated by IGF-I acting through the IGF-I receptor and does not involve IGF-II .
	manualset3
208149	5	417966	7	NULL	NULL	0	NULL	IGF-II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Estrogen-related proliferation in ROS17/2 .8 cells appears to be mediated by IGF-I acting through the IGF-I receptor and does not involve IGF-II .
	manualset3
208150	1	417967	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , our data suggest constitutive expression of shRNA results in accumulation of mature shRNA molecules , inducing cellular toxicity at late time points , despite the presence of gene silencing .
	manualset3
208151	2	417967	7	NULL	NULL	0	NULL	constitutive expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , our data suggest constitutive expression of shRNA results in accumulation of mature shRNA molecules , inducing cellular toxicity at late time points , despite the presence of gene silencing .
	manualset3
208152	3	417967	7	NULL	NULL	0	NULL	shRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , our data suggest constitutive expression of shRNA results in accumulation of mature shRNA molecules , inducing cellular toxicity at late time points , despite the presence of gene silencing .
	manualset3
208153	4	417967	7	NULL	NULL	0	NULL	accumulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , our data suggest constitutive expression of shRNA results in accumulation of mature shRNA molecules , inducing cellular toxicity at late time points , despite the presence of gene silencing .
	manualset3
208154	5	417967	7	NULL	NULL	0	NULL	mature shRNA molecules	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , our data suggest constitutive expression of shRNA results in accumulation of mature shRNA molecules , inducing cellular toxicity at late time points , despite the presence of gene silencing .
	manualset3
208155	6	417967	7	NULL	NULL	0	NULL	cellular toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , our data suggest constitutive expression of shRNA results in accumulation of mature shRNA molecules , inducing cellular toxicity at late time points , despite the presence of gene silencing .
	manualset3
208156	7	417967	7	NULL	NULL	0	NULL	 late time points	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , our data suggest constitutive expression of shRNA results in accumulation of mature shRNA molecules , inducing cellular toxicity at late time points , despite the presence of gene silencing .
	manualset3
208157	8	417967	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , our data suggest constitutive expression of shRNA results in accumulation of mature shRNA molecules , inducing cellular toxicity at late time points , despite the presence of gene silencing .
	manualset3
208158	9	417967	7	NULL	NULL	0	NULL	gene silencing	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , our data suggest constitutive expression of shRNA results in accumulation of mature shRNA molecules , inducing cellular toxicity at late time points , despite the presence of gene silencing .
	manualset3
208159	1	417968	7	NULL	NULL	0	NULL	Density shift experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Density shift experiments , in which the changes in buoyant density of membranes were studied after growth in deuterated media , showed no indication of large zones of conservation during membrane growth .
	manualset3
208160	2	417968	7	NULL	NULL	0	NULL	changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Density shift experiments , in which the changes in buoyant density of membranes were studied after growth in deuterated media , showed no indication of large zones of conservation during membrane growth .
	manualset3
208161	3	417968	7	NULL	NULL	0	NULL	buoyant density	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Density shift experiments , in which the changes in buoyant density of membranes were studied after growth in deuterated media , showed no indication of large zones of conservation during membrane growth .
	manualset3
208162	4	417968	7	NULL	NULL	0	NULL	membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Density shift experiments , in which the changes in buoyant density of membranes were studied after growth in deuterated media , showed no indication of large zones of conservation during membrane growth .
	manualset3
208163	5	417968	7	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Density shift experiments , in which the changes in buoyant density of membranes were studied after growth in deuterated media , showed no indication of large zones of conservation during membrane growth .
	manualset3
208164	6	417968	7	NULL	NULL	0	NULL	deuterated media	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Density shift experiments , in which the changes in buoyant density of membranes were studied after growth in deuterated media , showed no indication of large zones of conservation during membrane growth .
	manualset3
208165	7	417968	7	NULL	NULL	0	NULL	no indication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Density shift experiments , in which the changes in buoyant density of membranes were studied after growth in deuterated media , showed no indication of large zones of conservation during membrane growth .
	manualset3
208166	8	417968	7	NULL	NULL	0	NULL	 large zones of conservation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Density shift experiments , in which the changes in buoyant density of membranes were studied after growth in deuterated media , showed no indication of large zones of conservation during membrane growth .
	manualset3
208167	9	417968	7	NULL	NULL	0	NULL	membrane growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Density shift experiments , in which the changes in buoyant density of membranes were studied after growth in deuterated media , showed no indication of large zones of conservation during membrane growth .
	manualset3
208168	1	417969	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews different theoretical models concerning the prevention of substance use by adolescents .
	manualset3
208169	2	417969	7	NULL	NULL	0	NULL	different theoretical models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews different theoretical models concerning the prevention of substance use by adolescents .
	manualset3
208170	3	417969	7	NULL	NULL	0	NULL	prevention 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews different theoretical models concerning the prevention of substance use by adolescents .
	manualset3
208171	4	417969	7	NULL	NULL	0	NULL	substance use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews different theoretical models concerning the prevention of substance use by adolescents .
	manualset3
208172	5	417969	7	NULL	NULL	0	NULL	adolescents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews different theoretical models concerning the prevention of substance use by adolescents .
	manualset3
208173	1	417970	7	NULL	NULL	0	NULL	DCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine how DCs induce Th1 differentiation in the absence of IL-12 , we examined the response of IL-12-deficient DCs to bacterial lipopolysaccharide ( LPS ) .
	manualset3
208174	2	417970	7	NULL	NULL	0	NULL	Th1 differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine how DCs induce Th1 differentiation in the absence of IL-12 , we examined the response of IL-12-deficient DCs to bacterial lipopolysaccharide ( LPS ) .
	manualset3
208175	3	417970	7	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine how DCs induce Th1 differentiation in the absence of IL-12 , we examined the response of IL-12-deficient DCs to bacterial lipopolysaccharide ( LPS ) .
	manualset3
208176	4	417970	7	NULL	NULL	0	NULL	IL-12 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine how DCs induce Th1 differentiation in the absence of IL-12 , we examined the response of IL-12-deficient DCs to bacterial lipopolysaccharide ( LPS ) .
	manualset3
208177	5	417970	7	NULL	NULL	0	NULL	 response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine how DCs induce Th1 differentiation in the absence of IL-12 , we examined the response of IL-12-deficient DCs to bacterial lipopolysaccharide ( LPS ) .
	manualset3
208178	6	417970	7	NULL	NULL	0	NULL	IL-12-deficient DCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine how DCs induce Th1 differentiation in the absence of IL-12 , we examined the response of IL-12-deficient DCs to bacterial lipopolysaccharide ( LPS ) .
	manualset3
208179	7	417970	7	NULL	NULL	0	NULL	bacterial lipopolysaccharide ( LPS )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine how DCs induce Th1 differentiation in the absence of IL-12 , we examined the response of IL-12-deficient DCs to bacterial lipopolysaccharide ( LPS ) .
	manualset3
208180	1	417971	7	NULL	NULL	0	NULL	microinjection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Surprisingly , microinjection of Mdm2 mRNA in two-cell-stage embryos led to inhibition of cellular convergence during gastrulation .
	manualset3
208181	2	417971	7	NULL	NULL	0	NULL	Mdm2 mRNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Surprisingly , microinjection of Mdm2 mRNA in two-cell-stage embryos led to inhibition of cellular convergence during gastrulation .
	manualset3
208182	3	417971	7	NULL	NULL	0	NULL	two-cell-stage embryos	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Surprisingly , microinjection of Mdm2 mRNA in two-cell-stage embryos led to inhibition of cellular convergence during gastrulation .
	manualset3
208183	4	417971	7	NULL	NULL	0	NULL	inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Surprisingly , microinjection of Mdm2 mRNA in two-cell-stage embryos led to inhibition of cellular convergence during gastrulation .
	manualset3
208184	5	417971	7	NULL	NULL	0	NULL	cellular convergence 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Surprisingly , microinjection of Mdm2 mRNA in two-cell-stage embryos led to inhibition of cellular convergence during gastrulation .
	manualset3
208185	6	417971	7	NULL	NULL	0	NULL	gastrulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Surprisingly , microinjection of Mdm2 mRNA in two-cell-stage embryos led to inhibition of cellular convergence during gastrulation .
	manualset3
208186	1	417972	7	NULL	NULL	0	NULL	 intensified screening	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	With intensified screening and the use of new diagnostic tools for prostate cancer ( prostate-specific antigen , rectal ultrasound , magnetic resonance imaging with rectal coils , etc ) , the number of newly diagnosed cases of prostate cancer is rising rapidly , whereas the frequency of death due to prostate cancer remains almost stable .
	manualset3
208187	2	417972	7	NULL	NULL	NULL	NULL	new diagnostic tools	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	With intensified screening and the use of new diagnostic tools for prostate cancer ( prostate-specific antigen , rectal ultrasound , magnetic resonance imaging with rectal coils , etc ) , the number of newly diagnosed cases of prostate cancer is rising rapidly , whereas the frequency of death due to prostate cancer remains almost stable .
	manualset3
208188	3	417972	7	NULL	NULL	0	NULL	prostate cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	With intensified screening and the use of new diagnostic tools for prostate cancer ( prostate-specific antigen , rectal ultrasound , magnetic resonance imaging with rectal coils , etc ) , the number of newly diagnosed cases of prostate cancer is rising rapidly , whereas the frequency of death due to prostate cancer remains almost stable .
	manualset3
208189	4	417972	7	NULL	NULL	0	NULL	prostate-specific antigen	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	With intensified screening and the use of new diagnostic tools for prostate cancer ( prostate-specific antigen , rectal ultrasound , magnetic resonance imaging with rectal coils , etc ) , the number of newly diagnosed cases of prostate cancer is rising rapidly , whereas the frequency of death due to prostate cancer remains almost stable .
	manualset3
208190	5	417972	7	NULL	NULL	NULL	NULL	rectal ultrasound	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	With intensified screening and the use of new diagnostic tools for prostate cancer ( prostate-specific antigen , rectal ultrasound , magnetic resonance imaging with rectal coils , etc ) , the number of newly diagnosed cases of prostate cancer is rising rapidly , whereas the frequency of death due to prostate cancer remains almost stable .
	manualset3
208191	6	417972	7	NULL	NULL	NULL	NULL	magnetic resonance imaging  with rectal coils	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	With intensified screening and the use of new diagnostic tools for prostate cancer ( prostate-specific antigen , rectal ultrasound , magnetic resonance imaging with rectal coils , etc ) , the number of newly diagnosed cases of prostate cancer is rising rapidly , whereas the frequency of death due to prostate cancer remains almost stable .
	manualset3
208192	7	417972	7	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With intensified screening and the use of new diagnostic tools for prostate cancer ( prostate-specific antigen , rectal ultrasound , magnetic resonance imaging with rectal coils , etc ) , the number of newly diagnosed cases of prostate cancer is rising rapidly , whereas the frequency of death due to prostate cancer remains almost stable .
	manualset3
208193	8	417972	7	NULL	NULL	0	NULL	newly diagnosed cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	With intensified screening and the use of new diagnostic tools for prostate cancer ( prostate-specific antigen , rectal ultrasound , magnetic resonance imaging with rectal coils , etc ) , the number of newly diagnosed cases of prostate cancer is rising rapidly , whereas the frequency of death due to prostate cancer remains almost stable .
	manualset3
208194	9	417972	7	NULL	NULL	0	NULL	prostate cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	With intensified screening and the use of new diagnostic tools for prostate cancer ( prostate-specific antigen , rectal ultrasound , magnetic resonance imaging with rectal coils , etc ) , the number of newly diagnosed cases of prostate cancer is rising rapidly , whereas the frequency of death due to prostate cancer remains almost stable .
	manualset3
208195	10	417972	7	NULL	NULL	NULL	NULL	 frequency of death	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	With intensified screening and the use of new diagnostic tools for prostate cancer ( prostate-specific antigen , rectal ultrasound , magnetic resonance imaging with rectal coils , etc ) , the number of newly diagnosed cases of prostate cancer is rising rapidly , whereas the frequency of death due to prostate cancer remains almost stable .
	manualset3
208197	12	417972	7	NULL	NULL	0	NULL	prostate cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	With intensified screening and the use of new diagnostic tools for prostate cancer ( prostate-specific antigen , rectal ultrasound , magnetic resonance imaging with rectal coils , etc ) , the number of newly diagnosed cases of prostate cancer is rising rapidly , whereas the frequency of death due to prostate cancer remains almost stable .
	manualset3
208198	1	417973	7	NULL	NULL	0	NULL	Osteoblastoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Osteoblastoma of the spine ) .
	manualset3
208199	2	417973	7	NULL	NULL	0	NULL	spine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Osteoblastoma of the spine ) .
	manualset3
208200	1	417974	7	NULL	NULL	0	NULL	 TCM related contents	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	All the TCM related contents , such as physicians , medical works and official position of medicine etc. can be represented by the word .
	manualset3
208201	2	417974	7	NULL	NULL	0	NULL	physicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All the TCM related contents , such as physicians , medical works and official position of medicine etc. can be represented by the word .
	manualset3
208202	3	417974	7	NULL	NULL	0	NULL	medical works	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	All the TCM related contents , such as physicians , medical works and official position of medicine etc. can be represented by the word .
	manualset3
208203	4	417974	7	NULL	NULL	0	NULL	official position	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	All the TCM related contents , such as physicians , medical works and official position of medicine etc. can be represented by the word .
	manualset3
208204	5	417974	7	NULL	NULL	0	NULL	medicine	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	All the TCM related contents , such as physicians , medical works and official position of medicine etc. can be represented by the word .
	manualset3
208205	6	417974	7	NULL	NULL	0	NULL	word	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	All the TCM related contents , such as physicians , medical works and official position of medicine etc. can be represented by the word .
	manualset3
208206	1	417975	7	NULL	NULL	0	NULL	Thirty children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty children with autism were observed during their everyday school activities in order to examine patterns of spontaneous communication .
	manualset3
208207	2	417975	7	NULL	NULL	0	NULL	autism	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty children with autism were observed during their everyday school activities in order to examine patterns of spontaneous communication .
	manualset3
208208	3	417975	7	NULL	NULL	0	NULL	everyday school activities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty children with autism were observed during their everyday school activities in order to examine patterns of spontaneous communication .
	manualset3
208209	4	417975	7	NULL	NULL	0	NULL	patterns	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty children with autism were observed during their everyday school activities in order to examine patterns of spontaneous communication .
	manualset3
208210	5	417975	7	NULL	NULL	0	NULL	 spontaneous communication	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty children with autism were observed during their everyday school activities in order to examine patterns of spontaneous communication .
	manualset3
208211	1	417976	7	NULL	NULL	0	NULL	Dimerization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Dimerization is dependent upon disulphide bonding through an unpaired cysteine at position 67 .
	manualset3
208212	2	417976	7	NULL	NULL	0	NULL	disulphide bonding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dimerization is dependent upon disulphide bonding through an unpaired cysteine at position 67 .
	manualset3
208213	3	417976	7	NULL	NULL	0	NULL	unpaired cysteine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Dimerization is dependent upon disulphide bonding through an unpaired cysteine at position 67 .
	manualset3
208214	4	417976	7	NULL	NULL	0	NULL	position 67	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Dimerization is dependent upon disulphide bonding through an unpaired cysteine at position 67 .
	manualset3
208215	1	417977	7	NULL	NULL	NULL	NULL	extent of the injury	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The extent of the injury is directly related to the mucosal volume irradiated , anatomic subsite exposed , treatment intensity , and individual patient predisposition .
	manualset3
208217	3	417977	7	NULL	NULL	NULL	NULL	mucosal volume irradiated	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The extent of the injury is directly related to the mucosal volume irradiated , anatomic subsite exposed , treatment intensity , and individual patient predisposition .
	manualset3
208218	4	417977	7	NULL	NULL	0	NULL	anatomic subsite exposed	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The extent of the injury is directly related to the mucosal volume irradiated , anatomic subsite exposed , treatment intensity , and individual patient predisposition .
	manualset3
208219	5	417977	7	NULL	NULL	0	NULL	 treatment intensity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The extent of the injury is directly related to the mucosal volume irradiated , anatomic subsite exposed , treatment intensity , and individual patient predisposition .
	manualset3
208220	6	417977	7	NULL	NULL	NULL	NULL	 individual patient predisposition	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The extent of the injury is directly related to the mucosal volume irradiated , anatomic subsite exposed , treatment intensity , and individual patient predisposition .
	manualset3
208221	1	417978	7	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , the authors conclude that gene rearrangement analysis is a valuable tool in the study of diffuse mixed cell lymphomas and is complementary to immunophenotypic studies .
	manualset3
208222	2	417978	7	NULL	NULL	0	NULL	 gene rearrangement analysis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , the authors conclude that gene rearrangement analysis is a valuable tool in the study of diffuse mixed cell lymphomas and is complementary to immunophenotypic studies .
	manualset3
208223	3	417978	7	NULL	NULL	0	NULL	 valuable tool	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , the authors conclude that gene rearrangement analysis is a valuable tool in the study of diffuse mixed cell lymphomas and is complementary to immunophenotypic studies .
	manualset3
208224	4	417978	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , the authors conclude that gene rearrangement analysis is a valuable tool in the study of diffuse mixed cell lymphomas and is complementary to immunophenotypic studies .
	manualset3
208225	5	417978	7	NULL	NULL	0	NULL	diffuse mixed cell lymphomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , the authors conclude that gene rearrangement analysis is a valuable tool in the study of diffuse mixed cell lymphomas and is complementary to immunophenotypic studies .
	manualset3
208226	6	417978	7	NULL	NULL	0	NULL	immunophenotypic studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , the authors conclude that gene rearrangement analysis is a valuable tool in the study of diffuse mixed cell lymphomas and is complementary to immunophenotypic studies .
	manualset3
208227	1	417979	7	NULL	NULL	0	NULL	SMC ( 15 ) s	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	SMC ( 15 ) s can be classified into two major groups according to their length : small SMC ( 15 ) and large ones .
	manualset3
208228	2	417979	7	NULL	NULL	0	NULL	 two major groups	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	SMC ( 15 ) s can be classified into two major groups according to their length : small SMC ( 15 ) and large ones .
	manualset3
208229	3	417979	7	NULL	NULL	0	NULL	length	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	SMC ( 15 ) s can be classified into two major groups according to their length : small SMC ( 15 ) and large ones .
	manualset3
208230	4	417979	7	NULL	NULL	0	NULL	small SMC ( 15 )	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	SMC ( 15 ) s can be classified into two major groups according to their length : small SMC ( 15 ) and large ones .
	manualset3
208231	5	417979	7	NULL	NULL	0	NULL	large SMC ( 15 ) 	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	SMC ( 15 ) s can be classified into two major groups according to their length : small SMC ( 15 ) and large ones .
	manualset3
208232	1	417980	7	NULL	NULL	0	NULL	search 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A search of the genome sequence of this strain revealed the presence of a closely related orthologue ( TK2104 ) of bacterial DERA genes while no orthologue related to previously characterized PPM genes could be detected .
	manualset3
208233	2	417980	7	NULL	NULL	0	NULL	genome sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A search of the genome sequence of this strain revealed the presence of a closely related orthologue ( TK2104 ) of bacterial DERA genes while no orthologue related to previously characterized PPM genes could be detected .
	manualset3
208234	3	417980	7	NULL	NULL	0	NULL	strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A search of the genome sequence of this strain revealed the presence of a closely related orthologue ( TK2104 ) of bacterial DERA genes while no orthologue related to previously characterized PPM genes could be detected .
	manualset3
208235	4	417980	7	NULL	NULL	NULL	NULL	closely related orthologue TK2104 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A search of the genome sequence of this strain revealed the presence of a closely related orthologue ( TK2104 ) of bacterial DERA genes while no orthologue related to previously characterized PPM genes could be detected .
	manualset3
208236	5	417980	7	NULL	NULL	NULL	NULL	bacterial DERA genes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A search of the genome sequence of this strain revealed the presence of a closely related orthologue ( TK2104 ) of bacterial DERA genes while no orthologue related to previously characterized PPM genes could be detected .
	manualset3
208237	6	417980	7	NULL	NULL	0	NULL	no orthologue	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A search of the genome sequence of this strain revealed the presence of a closely related orthologue ( TK2104 ) of bacterial DERA genes while no orthologue related to previously characterized PPM genes could be detected .
	manualset3
208238	7	417980	7	NULL	NULL	0	NULL	PPM genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A search of the genome sequence of this strain revealed the presence of a closely related orthologue ( TK2104 ) of bacterial DERA genes while no orthologue related to previously characterized PPM genes could be detected .
	manualset3
208239	1	417981	7	NULL	NULL	0	NULL	surgical repair	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Delayed surgical repair of ruptured ligaments : a comparative biomechanical and histological study .
	manualset3
208240	2	417981	7	NULL	NULL	NULL	NULL	ruptured ligaments	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delayed surgical repair of ruptured ligaments : a comparative biomechanical and histological study .
	manualset3
208241	3	417981	7	NULL	NULL	0	NULL	biomechanical study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Delayed surgical repair of ruptured ligaments : a comparative biomechanical and histological study .
	manualset3
208242	4	417981	7	NULL	NULL	0	NULL	histological study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Delayed surgical repair of ruptured ligaments : a comparative biomechanical and histological study .
	manualset3
208243	1	417982	7	NULL	NULL	0	NULL	F ( 0 ) F ( 1 ) ATP synthase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The F ( 0 ) F ( 1 ) ATP synthase functions as a rotary motor where subunit rotation driven by a current of protons flowing through F ( 0 ) drives the binding changes in F ( 1 ) that are required for net ATP synthesis .
	manualset3
208244	2	417982	7	NULL	NULL	NULL	NULL	 rotary motor	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The F ( 0 ) F ( 1 ) ATP synthase functions as a rotary motor where subunit rotation driven by a current of protons flowing through F ( 0 ) drives the binding changes in F ( 1 ) that are required for net ATP synthesis .
	manualset3
208245	3	417982	7	NULL	NULL	NULL	NULL	subunit rotation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The F ( 0 ) F ( 1 ) ATP synthase functions as a rotary motor where subunit rotation driven by a current of protons flowing through F ( 0 ) drives the binding changes in F ( 1 ) that are required for net ATP synthesis .
	manualset3
208247	5	417982	7	NULL	NULL	NULL	NULL	current of protons	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The F ( 0 ) F ( 1 ) ATP synthase functions as a rotary motor where subunit rotation driven by a current of protons flowing through F ( 0 ) drives the binding changes in F ( 1 ) that are required for net ATP synthesis .
	manualset3
208248	6	417982	7	NULL	NULL	0	NULL	F ( 0 )	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The F ( 0 ) F ( 1 ) ATP synthase functions as a rotary motor where subunit rotation driven by a current of protons flowing through F ( 0 ) drives the binding changes in F ( 1 ) that are required for net ATP synthesis .
	manualset3
208249	7	417982	7	NULL	NULL	0	NULL	binding changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The F ( 0 ) F ( 1 ) ATP synthase functions as a rotary motor where subunit rotation driven by a current of protons flowing through F ( 0 ) drives the binding changes in F ( 1 ) that are required for net ATP synthesis .
	manualset3
208250	8	417982	7	NULL	NULL	0	NULL	F ( 1 )	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The F ( 0 ) F ( 1 ) ATP synthase functions as a rotary motor where subunit rotation driven by a current of protons flowing through F ( 0 ) drives the binding changes in F ( 1 ) that are required for net ATP synthesis .
	manualset3
208251	9	417982	7	NULL	NULL	0	NULL	ATP synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The F ( 0 ) F ( 1 ) ATP synthase functions as a rotary motor where subunit rotation driven by a current of protons flowing through F ( 0 ) drives the binding changes in F ( 1 ) that are required for net ATP synthesis .
	manualset3
208252	1	417983	7	NULL	NULL	0	NULL	Primary in-series palliation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary in-series palliation of hypoplastic left heart syndrome with mechanical lung assist in neonatal pigs .
	manualset3
208253	2	417983	7	NULL	NULL	0	NULL	hypoplastic left heart syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary in-series palliation of hypoplastic left heart syndrome with mechanical lung assist in neonatal pigs .
	manualset3
208254	3	417983	7	NULL	NULL	0	NULL	mechanical lung	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary in-series palliation of hypoplastic left heart syndrome with mechanical lung assist in neonatal pigs .
	manualset3
208255	4	417983	7	NULL	NULL	0	NULL	neonatal pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary in-series palliation of hypoplastic left heart syndrome with mechanical lung assist in neonatal pigs .
	manualset3
208256	1	417984	7	NULL	NULL	0	NULL	compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this compound is an analog of L-Phe and previous studies demonstrated a high affinity of this compound to large neutral amino acid transporter , the involvement of amino acid carriers did not appear to be significant in the Caco-2 cell model .
	manualset3
208257	2	417984	7	NULL	NULL	0	NULL	analog of L-Phe	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this compound is an analog of L-Phe and previous studies demonstrated a high affinity of this compound to large neutral amino acid transporter , the involvement of amino acid carriers did not appear to be significant in the Caco-2 cell model .
	manualset3
208258	3	417984	7	NULL	NULL	0	NULL	previous studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this compound is an analog of L-Phe and previous studies demonstrated a high affinity of this compound to large neutral amino acid transporter , the involvement of amino acid carriers did not appear to be significant in the Caco-2 cell model .
	manualset3
208259	4	417984	7	NULL	NULL	0	NULL	 high affinity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this compound is an analog of L-Phe and previous studies demonstrated a high affinity of this compound to large neutral amino acid transporter , the involvement of amino acid carriers did not appear to be significant in the Caco-2 cell model .
	manualset3
208260	5	417984	7	NULL	NULL	0	NULL	compound 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this compound is an analog of L-Phe and previous studies demonstrated a high affinity of this compound to large neutral amino acid transporter , the involvement of amino acid carriers did not appear to be significant in the Caco-2 cell model .
	manualset3
208261	6	417984	7	NULL	NULL	0	NULL	large neutral amino acid transporter	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this compound is an analog of L-Phe and previous studies demonstrated a high affinity of this compound to large neutral amino acid transporter , the involvement of amino acid carriers did not appear to be significant in the Caco-2 cell model .
	manualset3
208262	7	417984	7	NULL	NULL	0	NULL	 involvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this compound is an analog of L-Phe and previous studies demonstrated a high affinity of this compound to large neutral amino acid transporter , the involvement of amino acid carriers did not appear to be significant in the Caco-2 cell model .
	manualset3
208263	8	417984	7	NULL	NULL	0	NULL	amino acid carriers 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this compound is an analog of L-Phe and previous studies demonstrated a high affinity of this compound to large neutral amino acid transporter , the involvement of amino acid carriers did not appear to be significant in the Caco-2 cell model .
	manualset3
208264	9	417984	7	NULL	NULL	0	NULL	 Caco-2 cell model	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this compound is an analog of L-Phe and previous studies demonstrated a high affinity of this compound to large neutral amino acid transporter , the involvement of amino acid carriers did not appear to be significant in the Caco-2 cell model .
	manualset3
208265	1	417985	7	NULL	NULL	0	NULL	 knit-stitch 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The knit-stitch was preferred by 90 % of the surgeons .
	manualset3
208266	2	417985	7	NULL	NULL	0	NULL	90 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The knit-stitch was preferred by 90 % of the surgeons .
	manualset3
208267	3	417985	7	NULL	NULL	0	NULL	surgeons	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The knit-stitch was preferred by 90 % of the surgeons .
	manualset3
208268	1	417986	7	NULL	NULL	0	NULL	Cathepsin A 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Cathepsin A was purified from hog kidney with enzyme activity being monitored using both benzyloxycarbonyl-glutamyl-tyrosine ( ZGT ) and AI as substrates .
	manualset3
208269	2	417986	7	NULL	NULL	0	NULL	hog kidney	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Cathepsin A was purified from hog kidney with enzyme activity being monitored using both benzyloxycarbonyl-glutamyl-tyrosine ( ZGT ) and AI as substrates .
	manualset3
208270	3	417986	7	NULL	NULL	0	NULL	enzyme activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cathepsin A was purified from hog kidney with enzyme activity being monitored using both benzyloxycarbonyl-glutamyl-tyrosine ( ZGT ) and AI as substrates .
	manualset3
208271	4	417986	7	NULL	NULL	0	NULL	benzyloxycarbonyl-glutamyl-tyrosine ( ZGT )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Cathepsin A was purified from hog kidney with enzyme activity being monitored using both benzyloxycarbonyl-glutamyl-tyrosine ( ZGT ) and AI as substrates .
	manualset3
208272	5	417986	7	NULL	NULL	0	NULL	AI	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Cathepsin A was purified from hog kidney with enzyme activity being monitored using both benzyloxycarbonyl-glutamyl-tyrosine ( ZGT ) and AI as substrates .
	manualset3
208273	6	417986	7	NULL	NULL	0	NULL	substrates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Cathepsin A was purified from hog kidney with enzyme activity being monitored using both benzyloxycarbonyl-glutamyl-tyrosine ( ZGT ) and AI as substrates .
	manualset3
208274	1	417987	7	NULL	NULL	0	NULL	contradictory data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The contradictory data imply that it is inappropriate to conclude that suppressor cells are present at elevated levels in cancer patients by relying solely on the evidence of a depressed response to mitogens , either in a direct stimulation assay or in a coculture system .
	manualset3
208275	2	417987	7	NULL	NULL	0	NULL	suppressor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The contradictory data imply that it is inappropriate to conclude that suppressor cells are present at elevated levels in cancer patients by relying solely on the evidence of a depressed response to mitogens , either in a direct stimulation assay or in a coculture system .
	manualset3
208276	3	417987	7	NULL	NULL	0	NULL	 elevated levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The contradictory data imply that it is inappropriate to conclude that suppressor cells are present at elevated levels in cancer patients by relying solely on the evidence of a depressed response to mitogens , either in a direct stimulation assay or in a coculture system .
	manualset3
208277	4	417987	7	NULL	NULL	0	NULL	cancer patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The contradictory data imply that it is inappropriate to conclude that suppressor cells are present at elevated levels in cancer patients by relying solely on the evidence of a depressed response to mitogens , either in a direct stimulation assay or in a coculture system .
	manualset3
208278	5	417987	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The contradictory data imply that it is inappropriate to conclude that suppressor cells are present at elevated levels in cancer patients by relying solely on the evidence of a depressed response to mitogens , either in a direct stimulation assay or in a coculture system .
	manualset3
208279	6	417987	7	NULL	NULL	0	NULL	depressed response 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The contradictory data imply that it is inappropriate to conclude that suppressor cells are present at elevated levels in cancer patients by relying solely on the evidence of a depressed response to mitogens , either in a direct stimulation assay or in a coculture system .
	manualset3
208280	7	417987	7	NULL	NULL	0	NULL	mitogens	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The contradictory data imply that it is inappropriate to conclude that suppressor cells are present at elevated levels in cancer patients by relying solely on the evidence of a depressed response to mitogens , either in a direct stimulation assay or in a coculture system .
	manualset3
208281	8	417987	7	NULL	NULL	0	NULL	direct stimulation assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The contradictory data imply that it is inappropriate to conclude that suppressor cells are present at elevated levels in cancer patients by relying solely on the evidence of a depressed response to mitogens , either in a direct stimulation assay or in a coculture system .
	manualset3
208282	9	417987	7	NULL	NULL	0	NULL	coculture system	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The contradictory data imply that it is inappropriate to conclude that suppressor cells are present at elevated levels in cancer patients by relying solely on the evidence of a depressed response to mitogens , either in a direct stimulation assay or in a coculture system .
	manualset3
208283	1	417988	7	NULL	NULL	0	NULL	 chloroquine resistance locus	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The chloroquine resistance locus has been mapped to a 400 kilobase ( kb ) segment of chromosome 7 in a P. falciparum cross .
	manualset3
208284	2	417988	7	NULL	NULL	0	NULL	 400 kilobase ( kb ) segment 	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The chloroquine resistance locus has been mapped to a 400 kilobase ( kb ) segment of chromosome 7 in a P. falciparum cross .
	manualset3
208285	3	417988	7	NULL	NULL	0	NULL	chromosome 7 	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The chloroquine resistance locus has been mapped to a 400 kilobase ( kb ) segment of chromosome 7 in a P. falciparum cross .
	manualset3
208286	4	417988	7	NULL	NULL	0	NULL	P. falciparum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The chloroquine resistance locus has been mapped to a 400 kilobase ( kb ) segment of chromosome 7 in a P. falciparum cross .
	manualset3
208287	1	417989	7	NULL	NULL	0	NULL	calcium-independent PKC-epsilon inhibitor ( Ro31-8220 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A calcium-independent PKC-epsilon inhibitor ( Ro31-8220 ) , but not calcium-dependent PKC-alpha and - beta inhibitors , also blocked the PGD ( 2 ) effect on contraction , implying a role for a calcium-independent pathway .
	manualset3
208288	2	417989	7	NULL	NULL	0	NULL	calcium-dependent PKC-alpha inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A calcium-independent PKC-epsilon inhibitor ( Ro31-8220 ) , but not calcium-dependent PKC-alpha and - beta inhibitors , also blocked the PGD ( 2 ) effect on contraction , implying a role for a calcium-independent pathway .
	manualset3
208289	3	417989	7	NULL	NULL	0	NULL	calcium-dependent PKC-beta inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A calcium-independent PKC-epsilon inhibitor ( Ro31-8220 ) , but not calcium-dependent PKC-alpha and - beta inhibitors , also blocked the PGD ( 2 ) effect on contraction , implying a role for a calcium-independent pathway .
	manualset3
208290	4	417989	7	NULL	NULL	NULL	NULL	PGD ( 2 ) effect	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A calcium-independent PKC-epsilon inhibitor ( Ro31-8220 ) , but not calcium-dependent PKC-alpha and - beta inhibitors , also blocked the PGD ( 2 ) effect on contraction , implying a role for a calcium-independent pathway .
	manualset3
208291	5	417989	7	NULL	NULL	0	NULL	contraction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A calcium-independent PKC-epsilon inhibitor ( Ro31-8220 ) , but not calcium-dependent PKC-alpha and - beta inhibitors , also blocked the PGD ( 2 ) effect on contraction , implying a role for a calcium-independent pathway .
	manualset3
208292	6	417989	7	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A calcium-independent PKC-epsilon inhibitor ( Ro31-8220 ) , but not calcium-dependent PKC-alpha and - beta inhibitors , also blocked the PGD ( 2 ) effect on contraction , implying a role for a calcium-independent pathway .
	manualset3
208293	7	417989	7	NULL	NULL	0	NULL	calcium-independent pathway 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A calcium-independent PKC-epsilon inhibitor ( Ro31-8220 ) , but not calcium-dependent PKC-alpha and - beta inhibitors , also blocked the PGD ( 2 ) effect on contraction , implying a role for a calcium-independent pathway .
	manualset3
208294	1	417990	7	NULL	NULL	0	NULL	Central auditory processing	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Central auditory processing in schizophrenia patients with a history of auditory hallucinations has been reported to be impaired , and abnormalities of interhemispheric transfer have been implicated in these patients .
	manualset3
208295	2	417990	7	NULL	NULL	0	NULL	schizophrenia patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Central auditory processing in schizophrenia patients with a history of auditory hallucinations has been reported to be impaired , and abnormalities of interhemispheric transfer have been implicated in these patients .
	manualset3
208296	3	417990	7	NULL	NULL	0	NULL	 history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Central auditory processing in schizophrenia patients with a history of auditory hallucinations has been reported to be impaired , and abnormalities of interhemispheric transfer have been implicated in these patients .
	manualset3
208297	4	417990	7	NULL	NULL	0	NULL	auditory hallucinations 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Central auditory processing in schizophrenia patients with a history of auditory hallucinations has been reported to be impaired , and abnormalities of interhemispheric transfer have been implicated in these patients .
	manualset3
208298	5	417990	7	NULL	NULL	0	NULL	abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Central auditory processing in schizophrenia patients with a history of auditory hallucinations has been reported to be impaired , and abnormalities of interhemispheric transfer have been implicated in these patients .
	manualset3
208299	6	417990	7	NULL	NULL	0	NULL	interhemispheric transfer	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Central auditory processing in schizophrenia patients with a history of auditory hallucinations has been reported to be impaired , and abnormalities of interhemispheric transfer have been implicated in these patients .
	manualset3
208300	7	417990	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Central auditory processing in schizophrenia patients with a history of auditory hallucinations has been reported to be impaired , and abnormalities of interhemispheric transfer have been implicated in these patients .
	manualset3
208301	1	417991	7	NULL	NULL	0	NULL	 induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of 42A and 42C mRNAs and repression of S100 beta mRNA remained if nerve regeneration was prevented .
	manualset3
208302	2	417991	7	NULL	NULL	0	NULL	42A mRNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of 42A and 42C mRNAs and repression of S100 beta mRNA remained if nerve regeneration was prevented .
	manualset3
208303	3	417991	7	NULL	NULL	0	NULL	42C mRNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of 42A and 42C mRNAs and repression of S100 beta mRNA remained if nerve regeneration was prevented .
	manualset3
208304	4	417991	7	NULL	NULL	0	NULL	repression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of 42A and 42C mRNAs and repression of S100 beta mRNA remained if nerve regeneration was prevented .
	manualset3
208305	5	417991	7	NULL	NULL	0	NULL	S100 beta mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of 42A and 42C mRNAs and repression of S100 beta mRNA remained if nerve regeneration was prevented .
	manualset3
208306	6	417991	7	NULL	NULL	0	NULL	nerve regeneration 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of 42A and 42C mRNAs and repression of S100 beta mRNA remained if nerve regeneration was prevented .
	manualset3
208307	1	417992	7	NULL	NULL	0	NULL	 analyses 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	All the analyses revealed that the incorporation of the IF-WS2 altered significantly the crystallization behavior of PPS , in a way strongly dependent with the nanocomposite composition .
	manualset3
208308	2	417992	7	NULL	NULL	0	NULL	incorporation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	All the analyses revealed that the incorporation of the IF-WS2 altered significantly the crystallization behavior of PPS , in a way strongly dependent with the nanocomposite composition .
	manualset3
208309	3	417992	7	NULL	NULL	0	NULL	IF-WS2 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All the analyses revealed that the incorporation of the IF-WS2 altered significantly the crystallization behavior of PPS , in a way strongly dependent with the nanocomposite composition .
	manualset3
208310	4	417992	7	NULL	NULL	0	NULL	crystallization behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	All the analyses revealed that the incorporation of the IF-WS2 altered significantly the crystallization behavior of PPS , in a way strongly dependent with the nanocomposite composition .
	manualset3
208311	5	417992	7	NULL	NULL	0	NULL	PPS	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All the analyses revealed that the incorporation of the IF-WS2 altered significantly the crystallization behavior of PPS , in a way strongly dependent with the nanocomposite composition .
	manualset3
208312	6	417992	7	NULL	NULL	0	NULL	nanocomposite composition	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All the analyses revealed that the incorporation of the IF-WS2 altered significantly the crystallization behavior of PPS , in a way strongly dependent with the nanocomposite composition .
	manualset3
208313	1	417993	7	NULL	NULL	0	NULL	Gremlin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Gremlin plays a key role in the pathogenesis of pulmonary hypertension .
	manualset3
208314	2	417993	7	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gremlin plays a key role in the pathogenesis of pulmonary hypertension .
	manualset3
208315	3	417993	7	NULL	NULL	0	NULL	 pathogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gremlin plays a key role in the pathogenesis of pulmonary hypertension .
	manualset3
208316	4	417993	7	NULL	NULL	0	NULL	pulmonary hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gremlin plays a key role in the pathogenesis of pulmonary hypertension .
	manualset3
208317	1	417994	7	NULL	NULL	0	NULL	Inbred Carworth Farms Nelson ( CFN ) congenitally hyperlipidemic rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Inbred Carworth Farms Nelson ( CFN ) congenitally hyperlipidemic rats had significantly shorter coagulation and prothrombin times and higher levels of coagulation factors , II , V , VII , VIII , and X than did controls .
	manualset3
208318	2	417994	7	NULL	NULL	0	NULL	shorter coagulation time	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inbred Carworth Farms Nelson ( CFN ) congenitally hyperlipidemic rats had significantly shorter coagulation and prothrombin times and higher levels of coagulation factors , II , V , VII , VIII , and X than did controls .
	manualset3
208319	3	417994	7	NULL	NULL	0	NULL	prothrombin times	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inbred Carworth Farms Nelson ( CFN ) congenitally hyperlipidemic rats had significantly shorter coagulation and prothrombin times and higher levels of coagulation factors , II , V , VII , VIII , and X than did controls .
	manualset3
208320	4	417994	7	NULL	NULL	0	NULL	higher levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Inbred Carworth Farms Nelson ( CFN ) congenitally hyperlipidemic rats had significantly shorter coagulation and prothrombin times and higher levels of coagulation factors , II , V , VII , VIII , and X than did controls .
	manualset3
208321	5	417994	7	NULL	NULL	0	NULL	coagulation factors II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Inbred Carworth Farms Nelson ( CFN ) congenitally hyperlipidemic rats had significantly shorter coagulation and prothrombin times and higher levels of coagulation factors , II , V , VII , VIII , and X than did controls .
	manualset3
208322	6	417994	7	NULL	NULL	0	NULL	coagulation factors V	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Inbred Carworth Farms Nelson ( CFN ) congenitally hyperlipidemic rats had significantly shorter coagulation and prothrombin times and higher levels of coagulation factors , II , V , VII , VIII , and X than did controls .
	manualset3
208323	7	417994	7	NULL	NULL	0	NULL	coagulation factors VII	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Inbred Carworth Farms Nelson ( CFN ) congenitally hyperlipidemic rats had significantly shorter coagulation and prothrombin times and higher levels of coagulation factors , II , V , VII , VIII , and X than did controls .
	manualset3
208324	8	417994	7	NULL	NULL	0	NULL	coagulation factors VIII	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Inbred Carworth Farms Nelson ( CFN ) congenitally hyperlipidemic rats had significantly shorter coagulation and prothrombin times and higher levels of coagulation factors , II , V , VII , VIII , and X than did controls .
	manualset3
208325	9	417994	7	NULL	NULL	0	NULL	coagulation factors X	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Inbred Carworth Farms Nelson ( CFN ) congenitally hyperlipidemic rats had significantly shorter coagulation and prothrombin times and higher levels of coagulation factors , II , V , VII , VIII , and X than did controls .
	manualset3
208326	1	417995	7	NULL	NULL	0	NULL	Colonization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonization of Candida : prevalence among tongue-pierced and non-pierced immunocompetent adults .
	manualset3
208327	2	417995	7	NULL	NULL	0	NULL	Candida	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonization of Candida : prevalence among tongue-pierced and non-pierced immunocompetent adults .
	manualset3
208328	3	417995	7	NULL	NULL	0	NULL	tongue-pierced adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonization of Candida : prevalence among tongue-pierced and non-pierced immunocompetent adults .
	manualset3
208329	4	417995	7	NULL	NULL	0	NULL	non-pierced immunocompetent adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonization of Candida : prevalence among tongue-pierced and non-pierced immunocompetent adults .
	manualset3
208330	1	417996	7	NULL	NULL	0	NULL	Response speed 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Response speed was also remarkable ; equilibrium was attained within 5 minutes after addition of substrate DNA at 20 C .
	manualset3
208331	2	417996	7	NULL	NULL	0	NULL	equilibrium	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Response speed was also remarkable ; equilibrium was attained within 5 minutes after addition of substrate DNA at 20 C .
	manualset3
208332	3	417996	7	NULL	NULL	0	NULL	 5 minutes	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Response speed was also remarkable ; equilibrium was attained within 5 minutes after addition of substrate DNA at 20 C .
	manualset3
208333	4	417996	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Response speed was also remarkable ; equilibrium was attained within 5 minutes after addition of substrate DNA at 20 C .
	manualset3
208334	5	417996	7	NULL	NULL	0	NULL	substrate DNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Response speed was also remarkable ; equilibrium was attained within 5 minutes after addition of substrate DNA at 20 C .
	manualset3
208335	6	417996	7	NULL	NULL	0	NULL	20 C	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Response speed was also remarkable ; equilibrium was attained within 5 minutes after addition of substrate DNA at 20 C .
	manualset3
208336	1	417997	7	NULL	NULL	0	NULL	Heredity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Heredity in pathology of the mesenchyma ) .
	manualset3
208337	2	417997	7	NULL	NULL	0	NULL	 pathology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Heredity in pathology of the mesenchyma ) .
	manualset3
208338	3	417997	7	NULL	NULL	0	NULL	 mesenchyma	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	( Heredity in pathology of the mesenchyma ) .
	manualset3
208339	1	417998	7	NULL	NULL	0	NULL	Fludarabine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Fludarabine appears to be an effective initial induction therapy with a reasonable safety profile for patients with CLL .
	manualset3
208340	2	417998	7	NULL	NULL	0	NULL	initial induction therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Fludarabine appears to be an effective initial induction therapy with a reasonable safety profile for patients with CLL .
	manualset3
208341	3	417998	7	NULL	NULL	0	NULL	safety profile	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Fludarabine appears to be an effective initial induction therapy with a reasonable safety profile for patients with CLL .
	manualset3
208342	4	417998	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Fludarabine appears to be an effective initial induction therapy with a reasonable safety profile for patients with CLL .
	manualset3
208343	5	417998	7	NULL	NULL	0	NULL	 CLL	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Fludarabine appears to be an effective initial induction therapy with a reasonable safety profile for patients with CLL .
	manualset3
208344	1	417999	7	NULL	NULL	NULL	NULL	 catechins	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	All the assayed catechins inhibited plasma TBARS formation .
	manualset3
208345	2	417999	7	NULL	NULL	0	NULL	plasma TBARS formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All the assayed catechins inhibited plasma TBARS formation .
	manualset3
208346	1	418000	7	NULL	NULL	0	NULL	bursts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When the bursts were induced by perfusion with magnesium-free medium ( + / - ) -2 - APV was the more potent inhibitor ( ED50 66 microM for ( + / - ) -2 - APV and 110 microM for kynurenate ) .
	manualset3
208347	2	418000	7	NULL	NULL	0	NULL	perfusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When the bursts were induced by perfusion with magnesium-free medium ( + / - ) -2 - APV was the more potent inhibitor ( ED50 66 microM for ( + / - ) -2 - APV and 110 microM for kynurenate ) .
	manualset3
208348	3	418000	7	NULL	NULL	0	NULL	magnesium-free medium ( + / - ) -2 - APV	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	When the bursts were induced by perfusion with magnesium-free medium ( + / - ) -2 - APV was the more potent inhibitor ( ED50 66 microM for ( + / - ) -2 - APV and 110 microM for kynurenate ) .
	manualset3
208349	4	418000	7	NULL	NULL	0	NULL	potent inhibitor 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When the bursts were induced by perfusion with magnesium-free medium ( + / - ) -2 - APV was the more potent inhibitor ( ED50 66 microM for ( + / - ) -2 - APV and 110 microM for kynurenate ) .
	manualset3
208350	5	418000	7	NULL	NULL	0	NULL	ED50	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When the bursts were induced by perfusion with magnesium-free medium ( + / - ) -2 - APV was the more potent inhibitor ( ED50 66 microM for ( + / - ) -2 - APV and 110 microM for kynurenate ) .
	manualset3
208351	6	418000	7	NULL	NULL	0	NULL	 66 microM for ( + / - ) -2 - APV 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When the bursts were induced by perfusion with magnesium-free medium ( + / - ) -2 - APV was the more potent inhibitor ( ED50 66 microM for ( + / - ) -2 - APV and 110 microM for kynurenate ) .
	manualset3
208352	7	418000	7	NULL	NULL	0	NULL	110 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	When the bursts were induced by perfusion with magnesium-free medium ( + / - ) -2 - APV was the more potent inhibitor ( ED50 66 microM for ( + / - ) -2 - APV and 110 microM for kynurenate ) .
	manualset3
208353	8	418000	7	NULL	NULL	0	NULL	kynurenate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When the bursts were induced by perfusion with magnesium-free medium ( + / - ) -2 - APV was the more potent inhibitor ( ED50 66 microM for ( + / - ) -2 - APV and 110 microM for kynurenate ) .
	manualset3
208354	1	418001	7	NULL	NULL	0	NULL	Examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Examination of the gastric fundus with the fibergastroscope .
	manualset3
208355	2	418001	7	NULL	NULL	0	NULL	 gastric fundus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Examination of the gastric fundus with the fibergastroscope .
	manualset3
208356	3	418001	7	NULL	NULL	0	NULL	fibergastroscope 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Examination of the gastric fundus with the fibergastroscope .
	manualset3
208357	1	418002	7	NULL	NULL	0	NULL	Exercise testing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Exercise testing 3 h after the first dose showed a more marked ST-segment reduction by atenolol than by nebivolol ( 59 % vs. 18 % ) .
	manualset3
208358	2	418002	7	NULL	NULL	0	NULL	3 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Exercise testing 3 h after the first dose showed a more marked ST-segment reduction by atenolol than by nebivolol ( 59 % vs. 18 % ) .
	manualset3
208359	3	418002	7	NULL	NULL	0	NULL	 first dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Exercise testing 3 h after the first dose showed a more marked ST-segment reduction by atenolol than by nebivolol ( 59 % vs. 18 % ) .
	manualset3
208360	4	418002	7	NULL	NULL	0	NULL	 marked ST-segment reduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Exercise testing 3 h after the first dose showed a more marked ST-segment reduction by atenolol than by nebivolol ( 59 % vs. 18 % ) .
	manualset3
208361	5	418002	7	NULL	NULL	0	NULL	atenolol 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Exercise testing 3 h after the first dose showed a more marked ST-segment reduction by atenolol than by nebivolol ( 59 % vs. 18 % ) .
	manualset3
208362	6	418002	7	NULL	NULL	0	NULL	 nebivolol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Exercise testing 3 h after the first dose showed a more marked ST-segment reduction by atenolol than by nebivolol ( 59 % vs. 18 % ) .
	manualset3
208363	7	418002	7	NULL	NULL	0	NULL	59 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Exercise testing 3 h after the first dose showed a more marked ST-segment reduction by atenolol than by nebivolol ( 59 % vs. 18 % ) .
	manualset3
208364	8	418002	7	NULL	NULL	0	NULL	18 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Exercise testing 3 h after the first dose showed a more marked ST-segment reduction by atenolol than by nebivolol ( 59 % vs. 18 % ) .
	manualset3
208365	1	418003	7	NULL	NULL	0	NULL	metastatic disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This applies , however , only when metastatic disease is confined to the liver and when complete removal of the metastases is possible .
	manualset3
208366	2	418003	7	NULL	NULL	0	NULL	 liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This applies , however , only when metastatic disease is confined to the liver and when complete removal of the metastases is possible .
	manualset3
208367	3	418003	7	NULL	NULL	NULL	NULL	complete removal 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This applies , however , only when metastatic disease is confined to the liver and when complete removal of the metastases is possible .
	manualset3
208368	4	418003	7	NULL	NULL	NULL	NULL	metastases	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This applies , however , only when metastatic disease is confined to the liver and when complete removal of the metastases is possible .
	manualset3
208369	1	418004	7	NULL	NULL	0	NULL	Type 1 Diabetes ( T1D )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Type 1 Diabetes ( T1D ) , also called juvenile diabetes because of its classically early onset , is considered an autoimmune disease targeting the insulin-producing cells in the pancreatic islets of Langerhans .
	manualset3
208370	2	418004	7	NULL	NULL	0	NULL	juvenile diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Type 1 Diabetes ( T1D ) , also called juvenile diabetes because of its classically early onset , is considered an autoimmune disease targeting the insulin-producing cells in the pancreatic islets of Langerhans .
	manualset3
208371	3	418004	7	NULL	NULL	0	NULL	early onset 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Type 1 Diabetes ( T1D ) , also called juvenile diabetes because of its classically early onset , is considered an autoimmune disease targeting the insulin-producing cells in the pancreatic islets of Langerhans .
	manualset3
208372	4	418004	7	NULL	NULL	0	NULL	autoimmune disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Type 1 Diabetes ( T1D ) , also called juvenile diabetes because of its classically early onset , is considered an autoimmune disease targeting the insulin-producing cells in the pancreatic islets of Langerhans .
	manualset3
208373	5	418004	7	NULL	NULL	0	NULL	 insulin-producing cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Type 1 Diabetes ( T1D ) , also called juvenile diabetes because of its classically early onset , is considered an autoimmune disease targeting the insulin-producing cells in the pancreatic islets of Langerhans .
	manualset3
208374	6	418004	7	NULL	NULL	0	NULL	pancreatic islets of Langerhans 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Type 1 Diabetes ( T1D ) , also called juvenile diabetes because of its classically early onset , is considered an autoimmune disease targeting the insulin-producing cells in the pancreatic islets of Langerhans .
	manualset3
208375	1	418005	7	NULL	NULL	0	NULL	Labels	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Labels corresponded to 2 groups each of 3 group types ( i.e. , 2 intimacy groups , 2 task-oriented groups , and 2 social categories ) .
	manualset3
208376	2	418005	7	NULL	NULL	NULL	NULL	 2 groups	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Labels corresponded to 2 groups each of 3 group types ( i.e. , 2 intimacy groups , 2 task-oriented groups , and 2 social categories ) .
	manualset3
208377	3	418005	7	NULL	NULL	NULL	NULL	3 group types	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Labels corresponded to 2 groups each of 3 group types ( i.e. , 2 intimacy groups , 2 task-oriented groups , and 2 social categories ) .
	manualset3
208378	4	418005	7	NULL	NULL	0	NULL	 2 intimacy groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Labels corresponded to 2 groups each of 3 group types ( i.e. , 2 intimacy groups , 2 task-oriented groups , and 2 social categories ) .
	manualset3
208379	5	418005	7	NULL	NULL	0	NULL	2 task-oriented groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Labels corresponded to 2 groups each of 3 group types ( i.e. , 2 intimacy groups , 2 task-oriented groups , and 2 social categories ) .
	manualset3
208380	6	418005	7	NULL	NULL	0	NULL	 2 social categories 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Labels corresponded to 2 groups each of 3 group types ( i.e. , 2 intimacy groups , 2 task-oriented groups , and 2 social categories ) .
	manualset3
208381	1	418006	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	While in patients not undergoing CPB a tendency to the decrease of plasma thyroid hormones was observed during the early postoperative phase , in patients of the by-pass group a small increase was observed .
	manualset3
208382	2	418006	7	NULL	NULL	0	NULL	CPB	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	While in patients not undergoing CPB a tendency to the decrease of plasma thyroid hormones was observed during the early postoperative phase , in patients of the by-pass group a small increase was observed .
	manualset3
208383	3	418006	7	NULL	NULL	0	NULL	tendency 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While in patients not undergoing CPB a tendency to the decrease of plasma thyroid hormones was observed during the early postoperative phase , in patients of the by-pass group a small increase was observed .
	manualset3
208384	4	418006	7	NULL	NULL	0	NULL	decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While in patients not undergoing CPB a tendency to the decrease of plasma thyroid hormones was observed during the early postoperative phase , in patients of the by-pass group a small increase was observed .
	manualset3
208385	5	418006	7	NULL	NULL	0	NULL	plasma thyroid hormones	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While in patients not undergoing CPB a tendency to the decrease of plasma thyroid hormones was observed during the early postoperative phase , in patients of the by-pass group a small increase was observed .
	manualset3
208386	6	418006	7	NULL	NULL	0	NULL	early postoperative phase	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While in patients not undergoing CPB a tendency to the decrease of plasma thyroid hormones was observed during the early postoperative phase , in patients of the by-pass group a small increase was observed .
	manualset3
208387	7	418006	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	While in patients not undergoing CPB a tendency to the decrease of plasma thyroid hormones was observed during the early postoperative phase , in patients of the by-pass group a small increase was observed .
	manualset3
208388	8	418006	7	NULL	NULL	0	NULL	by-pass group 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	While in patients not undergoing CPB a tendency to the decrease of plasma thyroid hormones was observed during the early postoperative phase , in patients of the by-pass group a small increase was observed .
	manualset3
208389	9	418006	7	NULL	NULL	0	NULL	small increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While in patients not undergoing CPB a tendency to the decrease of plasma thyroid hormones was observed during the early postoperative phase , in patients of the by-pass group a small increase was observed .
	manualset3
208391	1	418007	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results may explain the 24-hour limitation of cold storage as well as its inferior results following ischemia injury .
	manualset3
208393	2	418007	7	NULL	NULL	0	NULL	24-hour 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	These results may explain the 24-hour limitation of cold storage as well as its inferior results following ischemia injury .
	manualset3
208399	3	418007	7	NULL	NULL	0	NULL	limitation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results may explain the 24-hour limitation of cold storage as well as its inferior results following ischemia injury .
	manualset3
208400	4	418007	7	NULL	NULL	0	NULL	cold storage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results may explain the 24-hour limitation of cold storage as well as its inferior results following ischemia injury .
	manualset3
208401	5	418007	7	NULL	NULL	0	NULL	inferior results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results may explain the 24-hour limitation of cold storage as well as its inferior results following ischemia injury .
	manualset3
208402	6	418007	7	NULL	NULL	0	NULL	ischemia injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results may explain the 24-hour limitation of cold storage as well as its inferior results following ischemia injury .
	manualset3
208403	1	418008	7	NULL	NULL	0	NULL	diabetic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All the diabetic patients in the study population had non-insulin dependent DM .
	manualset3
208404	2	418008	7	NULL	NULL	0	NULL	study population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All the diabetic patients in the study population had non-insulin dependent DM .
	manualset3
208405	3	418008	7	NULL	NULL	0	NULL	non-insulin dependent DM 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	All the diabetic patients in the study population had non-insulin dependent DM .
	manualset3
208437	1	418009	7	NULL	NULL	0	NULL	sequences	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the sequences around the start sites of DHFR and REP are not similar and our data suggest that they bind different proteins .
	manualset3
208438	2	418009	7	NULL	NULL	0	NULL	start sites	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the sequences around the start sites of DHFR and REP are not similar and our data suggest that they bind different proteins .
	manualset3
208439	3	418009	7	NULL	NULL	0	NULL	DHFR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the sequences around the start sites of DHFR and REP are not similar and our data suggest that they bind different proteins .
	manualset3
208440	4	418009	7	NULL	NULL	0	NULL	REP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the sequences around the start sites of DHFR and REP are not similar and our data suggest that they bind different proteins .
	manualset3
208441	5	418009	7	NULL	NULL	0	NULL	 data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the sequences around the start sites of DHFR and REP are not similar and our data suggest that they bind different proteins .
	manualset3
208442	6	418009	7	NULL	NULL	0	NULL	 proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the sequences around the start sites of DHFR and REP are not similar and our data suggest that they bind different proteins .
	manualset3
208443	1	418010	7	NULL	NULL	0	NULL	product	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	After digesting this product and the wild type taq-pET-15b plasmid with NheI and BamHI restriction enzymes , they were ligated and used for the transformation of E. coli DH5 competent cells .
	manualset3
208444	2	418010	7	NULL	NULL	0	NULL	wild type taq-pET-15b plasmid	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	After digesting this product and the wild type taq-pET-15b plasmid with NheI and BamHI restriction enzymes , they were ligated and used for the transformation of E. coli DH5 competent cells .
	manualset3
208445	3	418010	7	NULL	NULL	0	NULL	NheI restriction enzymes	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	After digesting this product and the wild type taq-pET-15b plasmid with NheI and BamHI restriction enzymes , they were ligated and used for the transformation of E. coli DH5 competent cells .
	manualset3
208446	4	418010	7	NULL	NULL	0	NULL	BamHI restriction enzymes	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	After digesting this product and the wild type taq-pET-15b plasmid with NheI and BamHI restriction enzymes , they were ligated and used for the transformation of E. coli DH5 competent cells .
	manualset3
208447	5	418010	7	NULL	NULL	0	NULL	 transformation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After digesting this product and the wild type taq-pET-15b plasmid with NheI and BamHI restriction enzymes , they were ligated and used for the transformation of E. coli DH5 competent cells .
	manualset3
208448	6	418010	7	NULL	NULL	0	NULL	E. coli DH5 competent cells .	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	After digesting this product and the wild type taq-pET-15b plasmid with NheI and BamHI restriction enzymes , they were ligated and used for the transformation of E. coli DH5 competent cells .
	manualset3
208449	1	418011	7	NULL	NULL	0	NULL	Interferon	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferon was incorporated in the microspheres at a high trapping efficiency , and the rate of interferon release from the microspheres was regulated by the extent of cross-linking with glutaraldehyde .
	manualset3
208450	2	418011	7	NULL	NULL	0	NULL	microspheres 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferon was incorporated in the microspheres at a high trapping efficiency , and the rate of interferon release from the microspheres was regulated by the extent of cross-linking with glutaraldehyde .
	manualset3
208451	3	418011	7	NULL	NULL	0	NULL	high trapping efficiency	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferon was incorporated in the microspheres at a high trapping efficiency , and the rate of interferon release from the microspheres was regulated by the extent of cross-linking with glutaraldehyde .
	manualset3
208452	4	418011	7	NULL	NULL	0	NULL	rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferon was incorporated in the microspheres at a high trapping efficiency , and the rate of interferon release from the microspheres was regulated by the extent of cross-linking with glutaraldehyde .
	manualset3
208453	5	418011	7	NULL	NULL	0	NULL	interferon release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferon was incorporated in the microspheres at a high trapping efficiency , and the rate of interferon release from the microspheres was regulated by the extent of cross-linking with glutaraldehyde .
	manualset3
208454	6	418011	7	NULL	NULL	0	NULL	 microspheres	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferon was incorporated in the microspheres at a high trapping efficiency , and the rate of interferon release from the microspheres was regulated by the extent of cross-linking with glutaraldehyde .
	manualset3
208455	7	418011	7	NULL	NULL	0	NULL	 extent 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferon was incorporated in the microspheres at a high trapping efficiency , and the rate of interferon release from the microspheres was regulated by the extent of cross-linking with glutaraldehyde .
	manualset3
208456	8	418011	7	NULL	NULL	0	NULL	cross-linking	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferon was incorporated in the microspheres at a high trapping efficiency , and the rate of interferon release from the microspheres was regulated by the extent of cross-linking with glutaraldehyde .
	manualset3
208457	9	418011	7	NULL	NULL	0	NULL	glutaraldehyde	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Interferon was incorporated in the microspheres at a high trapping efficiency , and the rate of interferon release from the microspheres was regulated by the extent of cross-linking with glutaraldehyde .
	manualset3
208458	1	418012	7	NULL	NULL	0	NULL	 distant sites	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All had distant sites of sepsis .
	manualset3
208459	2	418012	7	NULL	NULL	0	NULL	sepsis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All had distant sites of sepsis .
	manualset3
208460	1	418013	7	NULL	NULL	0	NULL	206 adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 206 adults who required either CT or DPL to assess possible abdominal injury , US was performed , before DPL or CT , and was aimed at the detection of intraperitoneal fluid .
	manualset3
208461	2	418013	7	NULL	NULL	0	NULL	CT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 206 adults who required either CT or DPL to assess possible abdominal injury , US was performed , before DPL or CT , and was aimed at the detection of intraperitoneal fluid .
	manualset3
208462	3	418013	7	NULL	NULL	0	NULL	DPL	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 206 adults who required either CT or DPL to assess possible abdominal injury , US was performed , before DPL or CT , and was aimed at the detection of intraperitoneal fluid .
	manualset3
208463	4	418013	7	NULL	NULL	0	NULL	 abdominal injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 206 adults who required either CT or DPL to assess possible abdominal injury , US was performed , before DPL or CT , and was aimed at the detection of intraperitoneal fluid .
	manualset3
208464	5	418013	7	NULL	NULL	0	NULL	US	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 206 adults who required either CT or DPL to assess possible abdominal injury , US was performed , before DPL or CT , and was aimed at the detection of intraperitoneal fluid .
	manualset3
208465	6	418013	7	NULL	NULL	0	NULL	DPL	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 206 adults who required either CT or DPL to assess possible abdominal injury , US was performed , before DPL or CT , and was aimed at the detection of intraperitoneal fluid .
	manualset3
208466	7	418013	7	NULL	NULL	0	NULL	CT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 206 adults who required either CT or DPL to assess possible abdominal injury , US was performed , before DPL or CT , and was aimed at the detection of intraperitoneal fluid .
	manualset3
208467	8	418013	7	NULL	NULL	0	NULL	detection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 206 adults who required either CT or DPL to assess possible abdominal injury , US was performed , before DPL or CT , and was aimed at the detection of intraperitoneal fluid .
	manualset3
208468	9	418013	7	NULL	NULL	0	NULL	intraperitoneal fluid	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In 206 adults who required either CT or DPL to assess possible abdominal injury , US was performed , before DPL or CT , and was aimed at the detection of intraperitoneal fluid .
	manualset3
208469	1	418014	7	NULL	NULL	0	NULL	 flavonoids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All the flavonoids tested acted as reversible inhibitors , and the quercetin-thrombin complex was found to be most stable at pH = 7.5 .
	manualset3
208470	2	418014	7	NULL	NULL	0	NULL	reversible inhibitors 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All the flavonoids tested acted as reversible inhibitors , and the quercetin-thrombin complex was found to be most stable at pH = 7.5 .
	manualset3
208471	3	418014	7	NULL	NULL	0	NULL	 quercetin-thrombin complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All the flavonoids tested acted as reversible inhibitors , and the quercetin-thrombin complex was found to be most stable at pH = 7.5 .
	manualset3
208472	4	418014	7	NULL	NULL	0	NULL	pH = 7.5	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All the flavonoids tested acted as reversible inhibitors , and the quercetin-thrombin complex was found to be most stable at pH = 7.5 .
	manualset3
208473	1	418015	7	NULL	NULL	0	NULL	CaCO3	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Both CaCO3 and vitamin D3 derivatives may be used in the prevention and treatment of renal bone disease .
	manualset3
208474	2	418015	7	NULL	NULL	0	NULL	vitamin D3 derivatives	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Both CaCO3 and vitamin D3 derivatives may be used in the prevention and treatment of renal bone disease .
	manualset3
208475	3	418015	7	NULL	NULL	NULL	NULL	prevention	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Both CaCO3 and vitamin D3 derivatives may be used in the prevention and treatment of renal bone disease .
	manualset3
208476	4	418015	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Both CaCO3 and vitamin D3 derivatives may be used in the prevention and treatment of renal bone disease .
	manualset3
208477	5	418015	7	NULL	NULL	0	NULL	renal bone disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Both CaCO3 and vitamin D3 derivatives may be used in the prevention and treatment of renal bone disease .
	manualset3
208478	1	418016	7	NULL	NULL	0	NULL	 role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the role of genetic polymorphisms of AhR related to the carcinogen metabolism and cell proliferation , genotypes of three AhR polymorphisms Ex1 +185 A ) G , IVS7 +33 T ) G and Ex10 +501 G ) A were determined in 616 lung cancer cases and 616 lung cancer-free controls .
	manualset3
208479	2	418016	7	NULL	NULL	0	NULL	genetic polymorphisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the role of genetic polymorphisms of AhR related to the carcinogen metabolism and cell proliferation , genotypes of three AhR polymorphisms Ex1 +185 A ) G , IVS7 +33 T ) G and Ex10 +501 G ) A were determined in 616 lung cancer cases and 616 lung cancer-free controls .
	manualset3
208480	3	418016	7	NULL	NULL	0	NULL	AhR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the role of genetic polymorphisms of AhR related to the carcinogen metabolism and cell proliferation , genotypes of three AhR polymorphisms Ex1 +185 A ) G , IVS7 +33 T ) G and Ex10 +501 G ) A were determined in 616 lung cancer cases and 616 lung cancer-free controls .
	manualset3
208481	4	418016	7	NULL	NULL	0	NULL	carcinogen metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the role of genetic polymorphisms of AhR related to the carcinogen metabolism and cell proliferation , genotypes of three AhR polymorphisms Ex1 +185 A ) G , IVS7 +33 T ) G and Ex10 +501 G ) A were determined in 616 lung cancer cases and 616 lung cancer-free controls .
	manualset3
208482	5	418016	7	NULL	NULL	0	NULL	cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the role of genetic polymorphisms of AhR related to the carcinogen metabolism and cell proliferation , genotypes of three AhR polymorphisms Ex1 +185 A ) G , IVS7 +33 T ) G and Ex10 +501 G ) A were determined in 616 lung cancer cases and 616 lung cancer-free controls .
	manualset3
208483	6	418016	7	NULL	NULL	0	NULL	genotypes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the role of genetic polymorphisms of AhR related to the carcinogen metabolism and cell proliferation , genotypes of three AhR polymorphisms Ex1 +185 A ) G , IVS7 +33 T ) G and Ex10 +501 G ) A were determined in 616 lung cancer cases and 616 lung cancer-free controls .
	manualset3
208484	7	418016	7	NULL	NULL	0	NULL	three AhR polymorphisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the role of genetic polymorphisms of AhR related to the carcinogen metabolism and cell proliferation , genotypes of three AhR polymorphisms Ex1 +185 A ) G , IVS7 +33 T ) G and Ex10 +501 G ) A were determined in 616 lung cancer cases and 616 lung cancer-free controls .
	manualset3
208485	8	418016	7	NULL	NULL	0	NULL	Ex1 +185 A ) G	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the role of genetic polymorphisms of AhR related to the carcinogen metabolism and cell proliferation , genotypes of three AhR polymorphisms Ex1 +185 A ) G , IVS7 +33 T ) G and Ex10 +501 G ) A were determined in 616 lung cancer cases and 616 lung cancer-free controls .
	manualset3
208486	9	418016	7	NULL	NULL	0	NULL	IVS7 +33 T ) G 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the role of genetic polymorphisms of AhR related to the carcinogen metabolism and cell proliferation , genotypes of three AhR polymorphisms Ex1 +185 A ) G , IVS7 +33 T ) G and Ex10 +501 G ) A were determined in 616 lung cancer cases and 616 lung cancer-free controls .
	manualset3
208487	10	418016	7	NULL	NULL	0	NULL	Ex10 +501 G ) A 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the role of genetic polymorphisms of AhR related to the carcinogen metabolism and cell proliferation , genotypes of three AhR polymorphisms Ex1 +185 A ) G , IVS7 +33 T ) G and Ex10 +501 G ) A were determined in 616 lung cancer cases and 616 lung cancer-free controls .
	manualset3
208488	11	418016	7	NULL	NULL	0	NULL	616 lung cancer cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the role of genetic polymorphisms of AhR related to the carcinogen metabolism and cell proliferation , genotypes of three AhR polymorphisms Ex1 +185 A ) G , IVS7 +33 T ) G and Ex10 +501 G ) A were determined in 616 lung cancer cases and 616 lung cancer-free controls .
	manualset3
208489	12	418016	7	NULL	NULL	0	NULL	616 lung cancer-free controls 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To evaluate the role of genetic polymorphisms of AhR related to the carcinogen metabolism and cell proliferation , genotypes of three AhR polymorphisms Ex1 +185 A ) G , IVS7 +33 T ) G and Ex10 +501 G ) A were determined in 616 lung cancer cases and 616 lung cancer-free controls .
	manualset3
208490	1	418017	7	NULL	NULL	0	NULL	MFH tumor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether MFH tumor cells actually express the features of histiocytes , i.e. , bone marrow-derived cells of monocyte-macrophage lineage , we studied the antigenic and enzymatic phenotype of 13 MFHs in situ using frozen and plastic sections , respectively .
	manualset3
208491	2	418017	7	NULL	NULL	0	NULL	 histiocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether MFH tumor cells actually express the features of histiocytes , i.e. , bone marrow-derived cells of monocyte-macrophage lineage , we studied the antigenic and enzymatic phenotype of 13 MFHs in situ using frozen and plastic sections , respectively .
	manualset3
208492	3	418017	7	NULL	NULL	0	NULL	 bone marrow-derived cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether MFH tumor cells actually express the features of histiocytes , i.e. , bone marrow-derived cells of monocyte-macrophage lineage , we studied the antigenic and enzymatic phenotype of 13 MFHs in situ using frozen and plastic sections , respectively .
	manualset3
208493	4	418017	7	NULL	NULL	0	NULL	monocyte-macrophage lineage	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether MFH tumor cells actually express the features of histiocytes , i.e. , bone marrow-derived cells of monocyte-macrophage lineage , we studied the antigenic and enzymatic phenotype of 13 MFHs in situ using frozen and plastic sections , respectively .
	manualset3
208494	5	418017	7	NULL	NULL	0	NULL	antigenic phenotype	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether MFH tumor cells actually express the features of histiocytes , i.e. , bone marrow-derived cells of monocyte-macrophage lineage , we studied the antigenic and enzymatic phenotype of 13 MFHs in situ using frozen and plastic sections , respectively .
	manualset3
208495	6	418017	7	NULL	NULL	0	NULL	enzymatic phenotype	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether MFH tumor cells actually express the features of histiocytes , i.e. , bone marrow-derived cells of monocyte-macrophage lineage , we studied the antigenic and enzymatic phenotype of 13 MFHs in situ using frozen and plastic sections , respectively .
	manualset3
208496	7	418017	7	NULL	NULL	NULL	NULL	13 MFHs 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To determine whether MFH tumor cells actually express the features of histiocytes , i.e. , bone marrow-derived cells of monocyte-macrophage lineage , we studied the antigenic and enzymatic phenotype of 13 MFHs in situ using frozen and plastic sections , respectively .
	manualset3
208497	8	418017	7	NULL	NULL	0	NULL	frozen and plastic sections 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether MFH tumor cells actually express the features of histiocytes , i.e. , bone marrow-derived cells of monocyte-macrophage lineage , we studied the antigenic and enzymatic phenotype of 13 MFHs in situ using frozen and plastic sections , respectively .
	manualset3
209233	9	418017	7	NULL	NULL	0	NULL	features	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To determine whether MFH tumor cells actually express the features of histiocytes , i.e. , bone marrow-derived cells of monocyte-macrophage lineage , we studied the antigenic and enzymatic phenotype of 13 MFHs in situ using frozen and plastic sections , respectively .
	manualset3
208498	1	418018	7	NULL	NULL	0	NULL	Faculty opinion	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Faculty and student opinion were similar and positive with respect to the use of the simulator and matching of educational objectives , its use as a learning experience , its use as an evaluation tool and the need for familiarity with the tool before use as an assessment method .
	manualset3
208499	2	418018	7	NULL	NULL	0	NULL	student opinion	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Faculty and student opinion were similar and positive with respect to the use of the simulator and matching of educational objectives , its use as a learning experience , its use as an evaluation tool and the need for familiarity with the tool before use as an assessment method .
	manualset3
208500	3	418018	7	NULL	NULL	0	NULL	simulator	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Faculty and student opinion were similar and positive with respect to the use of the simulator and matching of educational objectives , its use as a learning experience , its use as an evaluation tool and the need for familiarity with the tool before use as an assessment method .
	manualset3
208501	4	418018	7	NULL	NULL	0	NULL	matching	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Faculty and student opinion were similar and positive with respect to the use of the simulator and matching of educational objectives , its use as a learning experience , its use as an evaluation tool and the need for familiarity with the tool before use as an assessment method .
	manualset3
208502	5	418018	7	NULL	NULL	NULL	NULL	educational objectives	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Faculty and student opinion were similar and positive with respect to the use of the simulator and matching of educational objectives , its use as a learning experience , its use as an evaluation tool and the need for familiarity with the tool before use as an assessment method .
	manualset3
208503	6	418018	7	NULL	NULL	0	NULL	learning experience	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Faculty and student opinion were similar and positive with respect to the use of the simulator and matching of educational objectives , its use as a learning experience , its use as an evaluation tool and the need for familiarity with the tool before use as an assessment method .
	manualset3
208504	7	418018	7	NULL	NULL	NULL	NULL	evaluation tool	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Faculty and student opinion were similar and positive with respect to the use of the simulator and matching of educational objectives , its use as a learning experience , its use as an evaluation tool and the need for familiarity with the tool before use as an assessment method .
	manualset3
208505	8	418018	7	NULL	NULL	0	NULL	 tool 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Faculty and student opinion were similar and positive with respect to the use of the simulator and matching of educational objectives , its use as a learning experience , its use as an evaluation tool and the need for familiarity with the tool before use as an assessment method .
	manualset3
208506	9	418018	7	NULL	NULL	0	NULL	assessment method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Faculty and student opinion were similar and positive with respect to the use of the simulator and matching of educational objectives , its use as a learning experience , its use as an evaluation tool and the need for familiarity with the tool before use as an assessment method .
	manualset3
209234	10	418018	7	NULL	NULL	0	NULL	familiarity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Faculty and student opinion were similar and positive with respect to the use of the simulator and matching of educational objectives , its use as a learning experience , its use as an evaluation tool and the need for familiarity with the tool before use as an assessment method .
	manualset3
208507	1	418019	7	NULL	NULL	0	NULL	 cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The cells were also stimulated by IGF-1 alone , in the absence of exogenous competence factors .
	manualset3
208508	2	418019	7	NULL	NULL	0	NULL	 IGF-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The cells were also stimulated by IGF-1 alone , in the absence of exogenous competence factors .
	manualset3
208509	3	418019	7	NULL	NULL	0	NULL	absence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cells were also stimulated by IGF-1 alone , in the absence of exogenous competence factors .
	manualset3
208510	4	418019	7	NULL	NULL	0	NULL	exogenous competence factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cells were also stimulated by IGF-1 alone , in the absence of exogenous competence factors .
	manualset3
208511	1	418020	7	NULL	NULL	0	NULL	Measles	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Measles has the highest proportionate death rate of 13.1 % and it shares the highest fatality rate of 32.6 % with tetanus .
	manualset3
208512	2	418020	7	NULL	NULL	0	NULL	highest proportionate death rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measles has the highest proportionate death rate of 13.1 % and it shares the highest fatality rate of 32.6 % with tetanus .
	manualset3
208513	3	418020	7	NULL	NULL	0	NULL	13.1 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Measles has the highest proportionate death rate of 13.1 % and it shares the highest fatality rate of 32.6 % with tetanus .
	manualset3
208514	4	418020	7	NULL	NULL	0	NULL	highest fatality rate 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measles has the highest proportionate death rate of 13.1 % and it shares the highest fatality rate of 32.6 % with tetanus .
	manualset3
208515	5	418020	7	NULL	NULL	0	NULL	32.6 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Measles has the highest proportionate death rate of 13.1 % and it shares the highest fatality rate of 32.6 % with tetanus .
	manualset3
208516	6	418020	7	NULL	NULL	0	NULL	tetanus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Measles has the highest proportionate death rate of 13.1 % and it shares the highest fatality rate of 32.6 % with tetanus .
	manualset3
208517	1	418021	7	NULL	NULL	0	NULL	 Crusted scabies	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Crusted scabies at the spinal injury site of a paraplegic man ) .
	manualset3
208518	2	418021	7	NULL	NULL	0	NULL	spinal injury site	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Crusted scabies at the spinal injury site of a paraplegic man ) .
	manualset3
208519	3	418021	7	NULL	NULL	0	NULL	paraplegic man	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( Crusted scabies at the spinal injury site of a paraplegic man ) .
	manualset3
208520	1	418022	7	NULL	NULL	0	NULL	galactan - derived products	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All the galactan - and SPPP-derived products promoted the growth of probiotic strains of Bifidobacterium longum and Lactobacillus acidophilus and generally did not support the propagation of Clostridium perfringens in single culture fermentations .
	manualset3
208521	2	418022	7	NULL	NULL	0	NULL	SPPP-derived products	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All the galactan - and SPPP-derived products promoted the growth of probiotic strains of Bifidobacterium longum and Lactobacillus acidophilus and generally did not support the propagation of Clostridium perfringens in single culture fermentations .
	manualset3
208522	3	418022	7	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All the galactan - and SPPP-derived products promoted the growth of probiotic strains of Bifidobacterium longum and Lactobacillus acidophilus and generally did not support the propagation of Clostridium perfringens in single culture fermentations .
	manualset3
208523	4	418022	7	NULL	NULL	0	NULL	probiotic strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	All the galactan - and SPPP-derived products promoted the growth of probiotic strains of Bifidobacterium longum and Lactobacillus acidophilus and generally did not support the propagation of Clostridium perfringens in single culture fermentations .
	manualset3
208524	5	418022	7	NULL	NULL	0	NULL	Bifidobacterium longum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	All the galactan - and SPPP-derived products promoted the growth of probiotic strains of Bifidobacterium longum and Lactobacillus acidophilus and generally did not support the propagation of Clostridium perfringens in single culture fermentations .
	manualset3
208525	6	418022	7	NULL	NULL	0	NULL	Lactobacillus acidophilus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	All the galactan - and SPPP-derived products promoted the growth of probiotic strains of Bifidobacterium longum and Lactobacillus acidophilus and generally did not support the propagation of Clostridium perfringens in single culture fermentations .
	manualset3
208526	7	418022	7	NULL	NULL	0	NULL	propagation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All the galactan - and SPPP-derived products promoted the growth of probiotic strains of Bifidobacterium longum and Lactobacillus acidophilus and generally did not support the propagation of Clostridium perfringens in single culture fermentations .
	manualset3
208527	8	418022	7	NULL	NULL	0	NULL	Clostridium perfringens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	All the galactan - and SPPP-derived products promoted the growth of probiotic strains of Bifidobacterium longum and Lactobacillus acidophilus and generally did not support the propagation of Clostridium perfringens in single culture fermentations .
	manualset3
208528	9	418022	7	NULL	NULL	0	NULL	single culture fermentations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All the galactan - and SPPP-derived products promoted the growth of probiotic strains of Bifidobacterium longum and Lactobacillus acidophilus and generally did not support the propagation of Clostridium perfringens in single culture fermentations .
	manualset3
208529	1	418023	7	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the expression of bcl-2 has been examined in normal non-haematopoietic tissues , embryos , and psoriatic skin by immunohistochemical staining .
	manualset3
208530	2	418023	7	NULL	NULL	0	NULL	 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the expression of bcl-2 has been examined in normal non-haematopoietic tissues , embryos , and psoriatic skin by immunohistochemical staining .
	manualset3
208531	3	418023	7	NULL	NULL	0	NULL	 bcl-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the expression of bcl-2 has been examined in normal non-haematopoietic tissues , embryos , and psoriatic skin by immunohistochemical staining .
	manualset3
208532	4	418023	7	NULL	NULL	0	NULL	normal non-haematopoietic tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the expression of bcl-2 has been examined in normal non-haematopoietic tissues , embryos , and psoriatic skin by immunohistochemical staining .
	manualset3
208533	5	418023	7	NULL	NULL	0	NULL	embryos	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the expression of bcl-2 has been examined in normal non-haematopoietic tissues , embryos , and psoriatic skin by immunohistochemical staining .
	manualset3
208534	6	418023	7	NULL	NULL	0	NULL	 psoriatic skin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the expression of bcl-2 has been examined in normal non-haematopoietic tissues , embryos , and psoriatic skin by immunohistochemical staining .
	manualset3
208535	7	418023	7	NULL	NULL	0	NULL	immunohistochemical staining	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , the expression of bcl-2 has been examined in normal non-haematopoietic tissues , embryos , and psoriatic skin by immunohistochemical staining .
	manualset3
208536	1	418024	7	NULL	NULL	0	NULL	Non-macroglobulinaemic plasma cell dyscrasias	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Non-macroglobulinaemic plasma cell dyscrasias i hematological analysis in one-hundred cases ( author 's transl ) ) .
	manualset3
208537	2	418024	7	NULL	NULL	0	NULL	 i hematological analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Non-macroglobulinaemic plasma cell dyscrasias i hematological analysis in one-hundred cases ( author 's transl ) ) .
	manualset3
208538	3	418024	7	NULL	NULL	0	NULL	one-hundred cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Non-macroglobulinaemic plasma cell dyscrasias i hematological analysis in one-hundred cases ( author 's transl ) ) .
	manualset3
208539	4	418024	7	NULL	NULL	0	NULL	author 's transl	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Non-macroglobulinaemic plasma cell dyscrasias i hematological analysis in one-hundred cases ( author 's transl ) ) .
	manualset3
208540	1	418025	7	NULL	NULL	0	NULL	 Inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Inhibition of guinea pig sperm capacitation , the acrosome reaction and sperm-egg fusion by dl-propranolol in vitro ) .
	manualset3
208541	2	418025	7	NULL	NULL	0	NULL	guinea pig sperm capacitation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Inhibition of guinea pig sperm capacitation , the acrosome reaction and sperm-egg fusion by dl-propranolol in vitro ) .
	manualset3
208542	3	418025	7	NULL	NULL	0	NULL	acrosome reaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Inhibition of guinea pig sperm capacitation , the acrosome reaction and sperm-egg fusion by dl-propranolol in vitro ) .
	manualset3
208543	4	418025	7	NULL	NULL	0	NULL	sperm-egg fusion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Inhibition of guinea pig sperm capacitation , the acrosome reaction and sperm-egg fusion by dl-propranolol in vitro ) .
	manualset3
208544	5	418025	7	NULL	NULL	0	NULL	dl-propranolol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Inhibition of guinea pig sperm capacitation , the acrosome reaction and sperm-egg fusion by dl-propranolol in vitro ) .
	manualset3
208545	1	418026	7	NULL	NULL	0	NULL	 peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	These peptides represent a class of opioid receptor ligands that we have termed acetalins ( acetyl plus enkephalin ) .
	manualset3
208546	2	418026	7	NULL	NULL	0	NULL	class	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These peptides represent a class of opioid receptor ligands that we have termed acetalins ( acetyl plus enkephalin ) .
	manualset3
208547	3	418026	7	NULL	NULL	0	NULL	opioid receptor ligands	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	These peptides represent a class of opioid receptor ligands that we have termed acetalins ( acetyl plus enkephalin ) .
	manualset3
208548	4	418026	7	NULL	NULL	0	NULL	acetalins	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	These peptides represent a class of opioid receptor ligands that we have termed acetalins ( acetyl plus enkephalin ) .
	manualset3
208549	5	418026	7	NULL	NULL	0	NULL	acetyl plus enkephalin	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	These peptides represent a class of opioid receptor ligands that we have termed acetalins ( acetyl plus enkephalin ) .
	manualset3
208550	1	418027	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results further demonstrate the complex effects of AZT on erythropoiesis in vivo .
	manualset3
208551	2	418027	7	NULL	NULL	0	NULL	complex effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results further demonstrate the complex effects of AZT on erythropoiesis in vivo .
	manualset3
208552	3	418027	7	NULL	NULL	0	NULL	AZT	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These results further demonstrate the complex effects of AZT on erythropoiesis in vivo .
	manualset3
208553	4	418027	7	NULL	NULL	0	NULL	erythropoiesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results further demonstrate the complex effects of AZT on erythropoiesis in vivo .
	manualset3
208554	1	418028	7	NULL	NULL	0	NULL	steady state 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the steady state , where pO never decreased below the baseline , transient decreases occurred during the `` initial dip '' and `` poststimulus undershoot . ''
	manualset3
208555	2	418028	7	NULL	NULL	0	NULL	 pO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the steady state , where pO never decreased below the baseline , transient decreases occurred during the `` initial dip '' and `` poststimulus undershoot . ''
	manualset3
208556	3	418028	7	NULL	NULL	0	NULL	 baseline	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the steady state , where pO never decreased below the baseline , transient decreases occurred during the `` initial dip '' and `` poststimulus undershoot . ''
	manualset3
208557	4	418028	7	NULL	NULL	0	NULL	`` initial dip ''	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the steady state , where pO never decreased below the baseline , transient decreases occurred during the `` initial dip '' and `` poststimulus undershoot . ''
	manualset3
208558	5	418028	7	NULL	NULL	0	NULL	`` poststimulus undershoot . ''	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the steady state , where pO never decreased below the baseline , transient decreases occurred during the `` initial dip '' and `` poststimulus undershoot . ''
	manualset3
208559	1	418029	7	NULL	NULL	0	NULL	N-acetylaspartate levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	N-acetylaspartate and N-acetylaspartylglutamate levels in Alzheimer 's disease post-mortem brain tissue .
	manualset3
208560	2	418029	7	NULL	NULL	0	NULL	N-acetylaspartylglutamate levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	N-acetylaspartate and N-acetylaspartylglutamate levels in Alzheimer 's disease post-mortem brain tissue .
	manualset3
208561	3	418029	7	NULL	NULL	0	NULL	Alzheimer 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	N-acetylaspartate and N-acetylaspartylglutamate levels in Alzheimer 's disease post-mortem brain tissue .
	manualset3
208562	4	418029	7	NULL	NULL	0	NULL	post-mortem brain tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	N-acetylaspartate and N-acetylaspartylglutamate levels in Alzheimer 's disease post-mortem brain tissue .
	manualset3
208563	1	418030	7	NULL	NULL	0	NULL	Data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Data from this multicenter , phase II trial do not provide convincing evidence of CRC risk reduction from 6-month interventions with atorvastatin , sulindac , or ORAFTISynergy1 , although statistical power was limited by the relatively small sample size .
	manualset3
208564	2	418030	7	NULL	NULL	0	NULL	 multicenter	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Data from this multicenter , phase II trial do not provide convincing evidence of CRC risk reduction from 6-month interventions with atorvastatin , sulindac , or ORAFTISynergy1 , although statistical power was limited by the relatively small sample size .
	manualset3
208565	3	418030	7	NULL	NULL	0	NULL	phase II trial	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Data from this multicenter , phase II trial do not provide convincing evidence of CRC risk reduction from 6-month interventions with atorvastatin , sulindac , or ORAFTISynergy1 , although statistical power was limited by the relatively small sample size .
	manualset3
208566	4	418030	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Data from this multicenter , phase II trial do not provide convincing evidence of CRC risk reduction from 6-month interventions with atorvastatin , sulindac , or ORAFTISynergy1 , although statistical power was limited by the relatively small sample size .
	manualset3
208567	5	418030	7	NULL	NULL	0	NULL	CRC risk reduction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Data from this multicenter , phase II trial do not provide convincing evidence of CRC risk reduction from 6-month interventions with atorvastatin , sulindac , or ORAFTISynergy1 , although statistical power was limited by the relatively small sample size .
	manualset3
208568	6	418030	7	NULL	NULL	0	NULL	6-month interventions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Data from this multicenter , phase II trial do not provide convincing evidence of CRC risk reduction from 6-month interventions with atorvastatin , sulindac , or ORAFTISynergy1 , although statistical power was limited by the relatively small sample size .
	manualset3
208569	7	418030	7	NULL	NULL	0	NULL	atorvastatin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Data from this multicenter , phase II trial do not provide convincing evidence of CRC risk reduction from 6-month interventions with atorvastatin , sulindac , or ORAFTISynergy1 , although statistical power was limited by the relatively small sample size .
	manualset3
208570	8	418030	7	NULL	NULL	0	NULL	sulindac	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Data from this multicenter , phase II trial do not provide convincing evidence of CRC risk reduction from 6-month interventions with atorvastatin , sulindac , or ORAFTISynergy1 , although statistical power was limited by the relatively small sample size .
	manualset3
208571	9	418030	7	NULL	NULL	0	NULL	ORAFTISynergy1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Data from this multicenter , phase II trial do not provide convincing evidence of CRC risk reduction from 6-month interventions with atorvastatin , sulindac , or ORAFTISynergy1 , although statistical power was limited by the relatively small sample size .
	manualset3
208572	10	418030	7	NULL	NULL	0	NULL	statistical power	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Data from this multicenter , phase II trial do not provide convincing evidence of CRC risk reduction from 6-month interventions with atorvastatin , sulindac , or ORAFTISynergy1 , although statistical power was limited by the relatively small sample size .
	manualset3
208573	11	418030	7	NULL	NULL	0	NULL	small sample size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Data from this multicenter , phase II trial do not provide convincing evidence of CRC risk reduction from 6-month interventions with atorvastatin , sulindac , or ORAFTISynergy1 , although statistical power was limited by the relatively small sample size .
	manualset3
208574	1	418031	7	NULL	NULL	0	NULL	isolates	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All the isolates belonged to phylogenetic group A and to the ST23 complex .
	manualset3
208575	2	418031	7	NULL	NULL	0	NULL	phylogenetic group A	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	All the isolates belonged to phylogenetic group A and to the ST23 complex .
	manualset3
208576	3	418031	7	NULL	NULL	0	NULL	ST23 complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All the isolates belonged to phylogenetic group A and to the ST23 complex .
	manualset3
208577	1	418032	7	NULL	NULL	0	NULL	analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An analysis of the occurrences of errors along the dimensions of voicing and place showed that aphasics rarely produce utterances containing both voice and place substitutions .
	manualset3
208578	2	418032	7	NULL	NULL	0	NULL	 occurrences of errors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An analysis of the occurrences of errors along the dimensions of voicing and place showed that aphasics rarely produce utterances containing both voice and place substitutions .
	manualset3
208579	3	418032	7	NULL	NULL	NULL	NULL	dimensions of voicing and place	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An analysis of the occurrences of errors along the dimensions of voicing and place showed that aphasics rarely produce utterances containing both voice and place substitutions .
	manualset3
208580	4	418032	7	NULL	NULL	0	NULL	aphasics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An analysis of the occurrences of errors along the dimensions of voicing and place showed that aphasics rarely produce utterances containing both voice and place substitutions .
	manualset3
208581	5	418032	7	NULL	NULL	0	NULL	utterances 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An analysis of the occurrences of errors along the dimensions of voicing and place showed that aphasics rarely produce utterances containing both voice and place substitutions .
	manualset3
208582	6	418032	7	NULL	NULL	0	NULL	voice substitution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An analysis of the occurrences of errors along the dimensions of voicing and place showed that aphasics rarely produce utterances containing both voice and place substitutions .
	manualset3
208583	7	418032	7	NULL	NULL	0	NULL	place substitutions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An analysis of the occurrences of errors along the dimensions of voicing and place showed that aphasics rarely produce utterances containing both voice and place substitutions .
	manualset3
208585	1	418033	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , no expression of hGH-N or rGH would be expected in these cells .
	manualset3
208586	2	418033	7	NULL	NULL	0	NULL	hGH-N	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , no expression of hGH-N or rGH would be expected in these cells .
	manualset3
208587	3	418033	7	NULL	NULL	0	NULL	 rGH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , no expression of hGH-N or rGH would be expected in these cells .
	manualset3
208588	4	418033	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , no expression of hGH-N or rGH would be expected in these cells .
	manualset3
208589	1	418034	7	NULL	NULL	0	NULL	Cryptosporidiosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Cryptosporidiosis , caused by Cryptosporidium parvum , is life-threatening in individuals with compromised immune systems and a common serious primary cause of outbreaks of diarrhoea in newborn calves and goats .
	manualset3
208590	2	418034	7	NULL	NULL	0	NULL	Cryptosporidium parvum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Cryptosporidiosis , caused by Cryptosporidium parvum , is life-threatening in individuals with compromised immune systems and a common serious primary cause of outbreaks of diarrhoea in newborn calves and goats .
	manualset3
208591	3	418034	7	NULL	NULL	0	NULL	life-threatening	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Cryptosporidiosis , caused by Cryptosporidium parvum , is life-threatening in individuals with compromised immune systems and a common serious primary cause of outbreaks of diarrhoea in newborn calves and goats .
	manualset3
208592	4	418034	7	NULL	NULL	0	NULL	individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Cryptosporidiosis , caused by Cryptosporidium parvum , is life-threatening in individuals with compromised immune systems and a common serious primary cause of outbreaks of diarrhoea in newborn calves and goats .
	manualset3
208593	5	418034	7	NULL	NULL	0	NULL	compromised immune systems	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Cryptosporidiosis , caused by Cryptosporidium parvum , is life-threatening in individuals with compromised immune systems and a common serious primary cause of outbreaks of diarrhoea in newborn calves and goats .
	manualset3
208594	6	418034	7	NULL	NULL	0	NULL	serious primary cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Cryptosporidiosis , caused by Cryptosporidium parvum , is life-threatening in individuals with compromised immune systems and a common serious primary cause of outbreaks of diarrhoea in newborn calves and goats .
	manualset3
208595	7	418034	7	NULL	NULL	0	NULL	outbreaks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Cryptosporidiosis , caused by Cryptosporidium parvum , is life-threatening in individuals with compromised immune systems and a common serious primary cause of outbreaks of diarrhoea in newborn calves and goats .
	manualset3
208596	8	418034	7	NULL	NULL	NULL	NULL	diarrhoea	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cryptosporidiosis , caused by Cryptosporidium parvum , is life-threatening in individuals with compromised immune systems and a common serious primary cause of outbreaks of diarrhoea in newborn calves and goats .
	manualset3
208597	9	418034	7	NULL	NULL	0	NULL	newborn calves	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Cryptosporidiosis , caused by Cryptosporidium parvum , is life-threatening in individuals with compromised immune systems and a common serious primary cause of outbreaks of diarrhoea in newborn calves and goats .
	manualset3
208598	10	418034	7	NULL	NULL	0	NULL	 goats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Cryptosporidiosis , caused by Cryptosporidium parvum , is life-threatening in individuals with compromised immune systems and a common serious primary cause of outbreaks of diarrhoea in newborn calves and goats .
	manualset3
208599	1	418035	7	NULL	NULL	0	NULL	effects 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There also might be some effects of retinoic acid on the cAMP-dependent protein kinase that are unrelated to differentiation and to the presence of cRABP .
	manualset3
208600	2	418035	7	NULL	NULL	0	NULL	 retinoic acid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	There also might be some effects of retinoic acid on the cAMP-dependent protein kinase that are unrelated to differentiation and to the presence of cRABP .
	manualset3
208601	3	418035	7	NULL	NULL	0	NULL	 cAMP-dependent protein kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	There also might be some effects of retinoic acid on the cAMP-dependent protein kinase that are unrelated to differentiation and to the presence of cRABP .
	manualset3
208602	4	418035	7	NULL	NULL	0	NULL	 differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There also might be some effects of retinoic acid on the cAMP-dependent protein kinase that are unrelated to differentiation and to the presence of cRABP .
	manualset3
208603	5	418035	7	NULL	NULL	NULL	NULL	 presence 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There also might be some effects of retinoic acid on the cAMP-dependent protein kinase that are unrelated to differentiation and to the presence of cRABP .
	manualset3
208604	6	418035	7	NULL	NULL	0	NULL	cRABP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	There also might be some effects of retinoic acid on the cAMP-dependent protein kinase that are unrelated to differentiation and to the presence of cRABP .
	manualset3
208605	1	418036	7	NULL	NULL	0	NULL	Rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were euthanized 36 hours and 5 , 10 , and 15 days after infection , and hearts were collected for histology , mRNA , and protein analyses .
	manualset3
208606	2	418036	7	NULL	NULL	0	NULL	36 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were euthanized 36 hours and 5 , 10 , and 15 days after infection , and hearts were collected for histology , mRNA , and protein analyses .
	manualset3
208607	3	418036	7	NULL	NULL	0	NULL	5 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were euthanized 36 hours and 5 , 10 , and 15 days after infection , and hearts were collected for histology , mRNA , and protein analyses .
	manualset3
208608	4	418036	7	NULL	NULL	0	NULL	10 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were euthanized 36 hours and 5 , 10 , and 15 days after infection , and hearts were collected for histology , mRNA , and protein analyses .
	manualset3
208609	5	418036	7	NULL	NULL	0	NULL	15 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were euthanized 36 hours and 5 , 10 , and 15 days after infection , and hearts were collected for histology , mRNA , and protein analyses .
	manualset3
208610	6	418036	7	NULL	NULL	0	NULL	 infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were euthanized 36 hours and 5 , 10 , and 15 days after infection , and hearts were collected for histology , mRNA , and protein analyses .
	manualset3
208611	7	418036	7	NULL	NULL	0	NULL	hearts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were euthanized 36 hours and 5 , 10 , and 15 days after infection , and hearts were collected for histology , mRNA , and protein analyses .
	manualset3
208612	8	418036	7	NULL	NULL	0	NULL	histology	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were euthanized 36 hours and 5 , 10 , and 15 days after infection , and hearts were collected for histology , mRNA , and protein analyses .
	manualset3
208613	9	418036	7	NULL	NULL	0	NULL	mRNA analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were euthanized 36 hours and 5 , 10 , and 15 days after infection , and hearts were collected for histology , mRNA , and protein analyses .
	manualset3
208614	10	418036	7	NULL	NULL	0	NULL	protein analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were euthanized 36 hours and 5 , 10 , and 15 days after infection , and hearts were collected for histology , mRNA , and protein analyses .
	manualset3
208615	1	418037	7	NULL	NULL	0	NULL	statistical significance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No statistical significance was found between the dental and medical students ' scores , but there was a significant difference ( p = 0.006 ) in their perception of PBL curricula .
	manualset3
208616	2	418037	7	NULL	NULL	0	NULL	dental students scores	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	No statistical significance was found between the dental and medical students ' scores , but there was a significant difference ( p = 0.006 ) in their perception of PBL curricula .
	manualset3
208617	3	418037	7	NULL	NULL	0	NULL	medical students ' scores	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	No statistical significance was found between the dental and medical students ' scores , but there was a significant difference ( p = 0.006 ) in their perception of PBL curricula .
	manualset3
208618	4	418037	7	NULL	NULL	0	NULL	significant difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	No statistical significance was found between the dental and medical students ' scores , but there was a significant difference ( p = 0.006 ) in their perception of PBL curricula .
	manualset3
208619	5	418037	7	NULL	NULL	0	NULL	p = 0.006	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No statistical significance was found between the dental and medical students ' scores , but there was a significant difference ( p = 0.006 ) in their perception of PBL curricula .
	manualset3
208620	6	418037	7	NULL	NULL	0	NULL	perception	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No statistical significance was found between the dental and medical students ' scores , but there was a significant difference ( p = 0.006 ) in their perception of PBL curricula .
	manualset3
208621	7	418037	7	NULL	NULL	0	NULL	PBL curricula	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	No statistical significance was found between the dental and medical students ' scores , but there was a significant difference ( p = 0.006 ) in their perception of PBL curricula .
	manualset3
208622	1	418038	7	NULL	NULL	0	NULL	mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All the mutations generated displayed a decreased ability to transactivate the adenovirus E2 promoter .
	manualset3
208623	2	418038	7	NULL	NULL	NULL	NULL	 decreased ability 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	All the mutations generated displayed a decreased ability to transactivate the adenovirus E2 promoter .
	manualset3
208624	3	418038	7	NULL	NULL	0	NULL	adenovirus E2 promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	All the mutations generated displayed a decreased ability to transactivate the adenovirus E2 promoter .
	manualset3
208625	1	418039	7	NULL	NULL	0	NULL	Analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of receiver operating characteristic curves demonstrated that the outcome for patients with biopsies showing borderline change could be predicted with 90 % sensitivity and 79.1 % specificity using the optimal Foxp3 mRNA cutoff value .
	manualset3
208626	2	418039	7	NULL	NULL	0	NULL	receiver operating characteristic curves	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of receiver operating characteristic curves demonstrated that the outcome for patients with biopsies showing borderline change could be predicted with 90 % sensitivity and 79.1 % specificity using the optimal Foxp3 mRNA cutoff value .
	manualset3
208627	3	418039	7	NULL	NULL	0	NULL	 outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of receiver operating characteristic curves demonstrated that the outcome for patients with biopsies showing borderline change could be predicted with 90 % sensitivity and 79.1 % specificity using the optimal Foxp3 mRNA cutoff value .
	manualset3
208628	4	418039	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of receiver operating characteristic curves demonstrated that the outcome for patients with biopsies showing borderline change could be predicted with 90 % sensitivity and 79.1 % specificity using the optimal Foxp3 mRNA cutoff value .
	manualset3
208629	5	418039	7	NULL	NULL	0	NULL	biopsies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of receiver operating characteristic curves demonstrated that the outcome for patients with biopsies showing borderline change could be predicted with 90 % sensitivity and 79.1 % specificity using the optimal Foxp3 mRNA cutoff value .
	manualset3
208630	6	418039	7	NULL	NULL	0	NULL	borderline change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of receiver operating characteristic curves demonstrated that the outcome for patients with biopsies showing borderline change could be predicted with 90 % sensitivity and 79.1 % specificity using the optimal Foxp3 mRNA cutoff value .
	manualset3
208631	7	418039	7	NULL	NULL	0	NULL	 90 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of receiver operating characteristic curves demonstrated that the outcome for patients with biopsies showing borderline change could be predicted with 90 % sensitivity and 79.1 % specificity using the optimal Foxp3 mRNA cutoff value .
	manualset3
208632	8	418039	7	NULL	NULL	0	NULL	sensitivity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of receiver operating characteristic curves demonstrated that the outcome for patients with biopsies showing borderline change could be predicted with 90 % sensitivity and 79.1 % specificity using the optimal Foxp3 mRNA cutoff value .
	manualset3
208633	9	418039	7	NULL	NULL	0	NULL	79.1 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of receiver operating characteristic curves demonstrated that the outcome for patients with biopsies showing borderline change could be predicted with 90 % sensitivity and 79.1 % specificity using the optimal Foxp3 mRNA cutoff value .
	manualset3
208634	10	418039	7	NULL	NULL	0	NULL	specificity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of receiver operating characteristic curves demonstrated that the outcome for patients with biopsies showing borderline change could be predicted with 90 % sensitivity and 79.1 % specificity using the optimal Foxp3 mRNA cutoff value .
	manualset3
208635	11	418039	7	NULL	NULL	0	NULL	optimal Foxp3 mRNA cutoff value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of receiver operating characteristic curves demonstrated that the outcome for patients with biopsies showing borderline change could be predicted with 90 % sensitivity and 79.1 % specificity using the optimal Foxp3 mRNA cutoff value .
	manualset3
208636	1	418040	7	NULL	NULL	0	NULL	Bioassays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Bioassays with mosquito species ( Culex quinquefasciatus , Anopheles stephensi and Aedes aegypti ) and field trials were also satisfactory .
	manualset3
208637	2	418040	7	NULL	NULL	0	NULL	mosquito species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Bioassays with mosquito species ( Culex quinquefasciatus , Anopheles stephensi and Aedes aegypti ) and field trials were also satisfactory .
	manualset3
208638	3	418040	7	NULL	NULL	0	NULL	Culex quinquefasciatus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Bioassays with mosquito species ( Culex quinquefasciatus , Anopheles stephensi and Aedes aegypti ) and field trials were also satisfactory .
	manualset3
208639	4	418040	7	NULL	NULL	0	NULL	Anopheles stephensi	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Bioassays with mosquito species ( Culex quinquefasciatus , Anopheles stephensi and Aedes aegypti ) and field trials were also satisfactory .
	manualset3
208640	5	418040	7	NULL	NULL	0	NULL	Aedes aegypti 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Bioassays with mosquito species ( Culex quinquefasciatus , Anopheles stephensi and Aedes aegypti ) and field trials were also satisfactory .
	manualset3
208641	6	418040	7	NULL	NULL	0	NULL	field trials	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Bioassays with mosquito species ( Culex quinquefasciatus , Anopheles stephensi and Aedes aegypti ) and field trials were also satisfactory .
	manualset3
208642	1	418041	7	NULL	NULL	0	NULL	types	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , both types of enzymes were required for an effective defense against chemical oxidants that generate superoxide radicals and hydrogen peroxide .
	manualset3
208643	2	418041	7	NULL	NULL	0	NULL	enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , both types of enzymes were required for an effective defense against chemical oxidants that generate superoxide radicals and hydrogen peroxide .
	manualset3
208644	3	418041	7	NULL	NULL	0	NULL	defense	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , both types of enzymes were required for an effective defense against chemical oxidants that generate superoxide radicals and hydrogen peroxide .
	manualset3
208645	4	418041	7	NULL	NULL	0	NULL	chemical oxidants	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , both types of enzymes were required for an effective defense against chemical oxidants that generate superoxide radicals and hydrogen peroxide .
	manualset3
208646	5	418041	7	NULL	NULL	0	NULL	superoxide radicals	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	However , both types of enzymes were required for an effective defense against chemical oxidants that generate superoxide radicals and hydrogen peroxide .
	manualset3
208647	6	418041	7	NULL	NULL	0	NULL	hydrogen peroxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , both types of enzymes were required for an effective defense against chemical oxidants that generate superoxide radicals and hydrogen peroxide .
	manualset3
208648	1	418042	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All the patients were diagnosed as stage 3-4 endometriosis following laparoscopy .
	manualset3
208649	2	418042	7	NULL	NULL	0	NULL	stage 3-4	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All the patients were diagnosed as stage 3-4 endometriosis following laparoscopy .
	manualset3
208650	3	418042	7	NULL	NULL	NULL	NULL	endometriosis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	All the patients were diagnosed as stage 3-4 endometriosis following laparoscopy .
	manualset3
208651	4	418042	7	NULL	NULL	NULL	NULL	laparoscopy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	All the patients were diagnosed as stage 3-4 endometriosis following laparoscopy .
	manualset3
208652	1	418043	7	NULL	NULL	0	NULL	marker rescue strategies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using marker rescue and dominant interfering mutant strategies , we show that estrogen action via GPR30 promotes fibronectin ( FN ) matrix assembly by human breast cancer cells .
	manualset3
208653	2	418043	7	NULL	NULL	0	NULL	dominant interfering mutant strategies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using marker rescue and dominant interfering mutant strategies , we show that estrogen action via GPR30 promotes fibronectin ( FN ) matrix assembly by human breast cancer cells .
	manualset3
208654	3	418043	7	NULL	NULL	0	NULL	estrogen action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using marker rescue and dominant interfering mutant strategies , we show that estrogen action via GPR30 promotes fibronectin ( FN ) matrix assembly by human breast cancer cells .
	manualset3
208655	4	418043	7	NULL	NULL	0	NULL	GPR30	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using marker rescue and dominant interfering mutant strategies , we show that estrogen action via GPR30 promotes fibronectin ( FN ) matrix assembly by human breast cancer cells .
	manualset3
208656	5	418043	7	NULL	NULL	0	NULL	fibronectin ( FN ) matrix assembly	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using marker rescue and dominant interfering mutant strategies , we show that estrogen action via GPR30 promotes fibronectin ( FN ) matrix assembly by human breast cancer cells .
	manualset3
208657	6	418043	7	NULL	NULL	0	NULL	human breast cancer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using marker rescue and dominant interfering mutant strategies , we show that estrogen action via GPR30 promotes fibronectin ( FN ) matrix assembly by human breast cancer cells .
	manualset3
208658	1	418044	7	NULL	NULL	NULL	NULL	variable-velocity feature	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The variable-velocity feature allows low pedalling forces for individuals with very weak leg muscles , yet provides resistance to higher pedalling effort in stronger patients .
	manualset3
208659	2	418044	7	NULL	NULL	NULL	NULL	low pedalling forces	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The variable-velocity feature allows low pedalling forces for individuals with very weak leg muscles , yet provides resistance to higher pedalling effort in stronger patients .
	manualset3
208660	3	418044	7	NULL	NULL	0	NULL	individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The variable-velocity feature allows low pedalling forces for individuals with very weak leg muscles , yet provides resistance to higher pedalling effort in stronger patients .
	manualset3
208661	4	418044	7	NULL	NULL	0	NULL	very weak leg muscles 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The variable-velocity feature allows low pedalling forces for individuals with very weak leg muscles , yet provides resistance to higher pedalling effort in stronger patients .
	manualset3
208662	5	418044	7	NULL	NULL	0	NULL	higher pedalling effort	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The variable-velocity feature allows low pedalling forces for individuals with very weak leg muscles , yet provides resistance to higher pedalling effort in stronger patients .
	manualset3
208663	6	418044	7	NULL	NULL	0	NULL	stronger patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The variable-velocity feature allows low pedalling forces for individuals with very weak leg muscles , yet provides resistance to higher pedalling effort in stronger patients .
	manualset3
208664	7	418044	7	NULL	NULL	0	NULL	resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The variable-velocity feature allows low pedalling forces for individuals with very weak leg muscles , yet provides resistance to higher pedalling effort in stronger patients .
	manualset3
208665	1	418045	7	NULL	NULL	0	NULL	 results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results represent a conceptual advance in understanding a potential molecular basis for initiation of autoimmunity in systemic lupus erythematosus .
	manualset3
208666	2	418045	7	NULL	NULL	0	NULL	conceptual advance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results represent a conceptual advance in understanding a potential molecular basis for initiation of autoimmunity in systemic lupus erythematosus .
	manualset3
208667	3	418045	7	NULL	NULL	0	NULL	potential molecular basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results represent a conceptual advance in understanding a potential molecular basis for initiation of autoimmunity in systemic lupus erythematosus .
	manualset3
208668	4	418045	7	NULL	NULL	0	NULL	 initiation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results represent a conceptual advance in understanding a potential molecular basis for initiation of autoimmunity in systemic lupus erythematosus .
	manualset3
208669	5	418045	7	NULL	NULL	0	NULL	autoimmunity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results represent a conceptual advance in understanding a potential molecular basis for initiation of autoimmunity in systemic lupus erythematosus .
	manualset3
208670	6	418045	7	NULL	NULL	0	NULL	systemic lupus erythematosus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The results represent a conceptual advance in understanding a potential molecular basis for initiation of autoimmunity in systemic lupus erythematosus .
	manualset3
209816	7	418045	7	NULL	NULL	0	NULL	understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results represent a conceptual advance in understanding a potential molecular basis for initiation of autoimmunity in systemic lupus erythematosus .
	manualset3
208671	1	418046	7	NULL	NULL	0	NULL	Domains	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Domains of physical function were not consistently related to domains of HRQOL .
	manualset3
208672	2	418046	7	NULL	NULL	0	NULL	physical function 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Domains of physical function were not consistently related to domains of HRQOL .
	manualset3
208673	3	418046	7	NULL	NULL	0	NULL	domains	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Domains of physical function were not consistently related to domains of HRQOL .
	manualset3
208674	4	418046	7	NULL	NULL	0	NULL	HRQOL	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Domains of physical function were not consistently related to domains of HRQOL .
	manualset3
208675	1	418047	7	NULL	NULL	0	NULL	Alpha acid glycoprotein binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Alpha acid glycoprotein binding is discussed as a potential factor to influence drug tissue distribution , and it is concluded that there is reasonable evidence that for tamsulosin this mechanism is responsible for the difference in free fraction of the drug observed in plasma and prostate , which could contribute to its relative absence of blood pressure effects in patients with LUT symptoms related to benign prostate hyperplasia ( LUTS-BPH ) .
	manualset3
208676	2	418047	7	NULL	NULL	0	NULL	 potential factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Alpha acid glycoprotein binding is discussed as a potential factor to influence drug tissue distribution , and it is concluded that there is reasonable evidence that for tamsulosin this mechanism is responsible for the difference in free fraction of the drug observed in plasma and prostate , which could contribute to its relative absence of blood pressure effects in patients with LUT symptoms related to benign prostate hyperplasia ( LUTS-BPH ) .
	manualset3
208677	3	418047	7	NULL	NULL	0	NULL	drug tissue distribution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Alpha acid glycoprotein binding is discussed as a potential factor to influence drug tissue distribution , and it is concluded that there is reasonable evidence that for tamsulosin this mechanism is responsible for the difference in free fraction of the drug observed in plasma and prostate , which could contribute to its relative absence of blood pressure effects in patients with LUT symptoms related to benign prostate hyperplasia ( LUTS-BPH ) .
	manualset3
208678	4	418047	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Alpha acid glycoprotein binding is discussed as a potential factor to influence drug tissue distribution , and it is concluded that there is reasonable evidence that for tamsulosin this mechanism is responsible for the difference in free fraction of the drug observed in plasma and prostate , which could contribute to its relative absence of blood pressure effects in patients with LUT symptoms related to benign prostate hyperplasia ( LUTS-BPH ) .
	manualset3
208679	5	418047	7	NULL	NULL	0	NULL	tamsulosin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Alpha acid glycoprotein binding is discussed as a potential factor to influence drug tissue distribution , and it is concluded that there is reasonable evidence that for tamsulosin this mechanism is responsible for the difference in free fraction of the drug observed in plasma and prostate , which could contribute to its relative absence of blood pressure effects in patients with LUT symptoms related to benign prostate hyperplasia ( LUTS-BPH ) .
	manualset3
208680	6	418047	7	NULL	NULL	0	NULL	mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Alpha acid glycoprotein binding is discussed as a potential factor to influence drug tissue distribution , and it is concluded that there is reasonable evidence that for tamsulosin this mechanism is responsible for the difference in free fraction of the drug observed in plasma and prostate , which could contribute to its relative absence of blood pressure effects in patients with LUT symptoms related to benign prostate hyperplasia ( LUTS-BPH ) .
	manualset3
208681	7	418047	7	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Alpha acid glycoprotein binding is discussed as a potential factor to influence drug tissue distribution , and it is concluded that there is reasonable evidence that for tamsulosin this mechanism is responsible for the difference in free fraction of the drug observed in plasma and prostate , which could contribute to its relative absence of blood pressure effects in patients with LUT symptoms related to benign prostate hyperplasia ( LUTS-BPH ) .
	manualset3
208682	8	418047	7	NULL	NULL	0	NULL	free fraction	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Alpha acid glycoprotein binding is discussed as a potential factor to influence drug tissue distribution , and it is concluded that there is reasonable evidence that for tamsulosin this mechanism is responsible for the difference in free fraction of the drug observed in plasma and prostate , which could contribute to its relative absence of blood pressure effects in patients with LUT symptoms related to benign prostate hyperplasia ( LUTS-BPH ) .
	manualset3
208683	9	418047	7	NULL	NULL	0	NULL	drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Alpha acid glycoprotein binding is discussed as a potential factor to influence drug tissue distribution , and it is concluded that there is reasonable evidence that for tamsulosin this mechanism is responsible for the difference in free fraction of the drug observed in plasma and prostate , which could contribute to its relative absence of blood pressure effects in patients with LUT symptoms related to benign prostate hyperplasia ( LUTS-BPH ) .
	manualset3
208684	10	418047	7	NULL	NULL	0	NULL	plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Alpha acid glycoprotein binding is discussed as a potential factor to influence drug tissue distribution , and it is concluded that there is reasonable evidence that for tamsulosin this mechanism is responsible for the difference in free fraction of the drug observed in plasma and prostate , which could contribute to its relative absence of blood pressure effects in patients with LUT symptoms related to benign prostate hyperplasia ( LUTS-BPH ) .
	manualset3
208685	11	418047	7	NULL	NULL	0	NULL	prostate	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Alpha acid glycoprotein binding is discussed as a potential factor to influence drug tissue distribution , and it is concluded that there is reasonable evidence that for tamsulosin this mechanism is responsible for the difference in free fraction of the drug observed in plasma and prostate , which could contribute to its relative absence of blood pressure effects in patients with LUT symptoms related to benign prostate hyperplasia ( LUTS-BPH ) .
	manualset3
208686	12	418047	7	NULL	NULL	0	NULL	relative absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Alpha acid glycoprotein binding is discussed as a potential factor to influence drug tissue distribution , and it is concluded that there is reasonable evidence that for tamsulosin this mechanism is responsible for the difference in free fraction of the drug observed in plasma and prostate , which could contribute to its relative absence of blood pressure effects in patients with LUT symptoms related to benign prostate hyperplasia ( LUTS-BPH ) .
	manualset3
208687	13	418047	7	NULL	NULL	NULL	NULL	blood pressure effects	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Alpha acid glycoprotein binding is discussed as a potential factor to influence drug tissue distribution , and it is concluded that there is reasonable evidence that for tamsulosin this mechanism is responsible for the difference in free fraction of the drug observed in plasma and prostate , which could contribute to its relative absence of blood pressure effects in patients with LUT symptoms related to benign prostate hyperplasia ( LUTS-BPH ) .
	manualset3
208688	14	418047	7	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Alpha acid glycoprotein binding is discussed as a potential factor to influence drug tissue distribution , and it is concluded that there is reasonable evidence that for tamsulosin this mechanism is responsible for the difference in free fraction of the drug observed in plasma and prostate , which could contribute to its relative absence of blood pressure effects in patients with LUT symptoms related to benign prostate hyperplasia ( LUTS-BPH ) .
	manualset3
208689	15	418047	7	NULL	NULL	NULL	NULL	LUT symptoms	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Alpha acid glycoprotein binding is discussed as a potential factor to influence drug tissue distribution , and it is concluded that there is reasonable evidence that for tamsulosin this mechanism is responsible for the difference in free fraction of the drug observed in plasma and prostate , which could contribute to its relative absence of blood pressure effects in patients with LUT symptoms related to benign prostate hyperplasia ( LUTS-BPH ) .
	manualset3
208690	16	418047	7	NULL	NULL	0	NULL	benign prostate hyperplasia ( LUTS-BPH )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Alpha acid glycoprotein binding is discussed as a potential factor to influence drug tissue distribution , and it is concluded that there is reasonable evidence that for tamsulosin this mechanism is responsible for the difference in free fraction of the drug observed in plasma and prostate , which could contribute to its relative absence of blood pressure effects in patients with LUT symptoms related to benign prostate hyperplasia ( LUTS-BPH ) .
	manualset3
208691	1	418048	7	NULL	NULL	0	NULL	brain concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The brain concentration of the prominent 27-mer metabolite is greater than that observed in the lung or spleen .
	manualset3
208692	2	418048	7	NULL	NULL	0	NULL	27-mer metabolite	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The brain concentration of the prominent 27-mer metabolite is greater than that observed in the lung or spleen .
	manualset3
208693	3	418048	7	NULL	NULL	0	NULL	 lung	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The brain concentration of the prominent 27-mer metabolite is greater than that observed in the lung or spleen .
	manualset3
208694	4	418048	7	NULL	NULL	0	NULL	 spleen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The brain concentration of the prominent 27-mer metabolite is greater than that observed in the lung or spleen .
	manualset3
208695	1	418049	7	NULL	NULL	NULL	NULL	sensitivity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The sensitivity of coho to Polyphase P-100 was altered by their developmental stage .
	manualset3
208696	2	418049	7	NULL	NULL	0	NULL	coho	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity of coho to Polyphase P-100 was altered by their developmental stage .
	manualset3
208697	3	418049	7	NULL	NULL	0	NULL	Polyphase P-100	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity of coho to Polyphase P-100 was altered by their developmental stage .
	manualset3
208698	4	418049	7	NULL	NULL	0	NULL	developmental stage 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The sensitivity of coho to Polyphase P-100 was altered by their developmental stage .
	manualset3
208699	1	418050	7	NULL	NULL	0	NULL	Lenses	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Lenses that translate as a whole , in shark , bony fish and frog , showed stress fibers ( SFs ) at the basal or apical end of the cells .
	manualset3
208700	2	418050	7	NULL	NULL	0	NULL	shark	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Lenses that translate as a whole , in shark , bony fish and frog , showed stress fibers ( SFs ) at the basal or apical end of the cells .
	manualset3
208701	3	418050	7	NULL	NULL	0	NULL	bony fish	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Lenses that translate as a whole , in shark , bony fish and frog , showed stress fibers ( SFs ) at the basal or apical end of the cells .
	manualset3
208702	4	418050	7	NULL	NULL	0	NULL	 frog	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Lenses that translate as a whole , in shark , bony fish and frog , showed stress fibers ( SFs ) at the basal or apical end of the cells .
	manualset3
208703	5	418050	7	NULL	NULL	NULL	NULL	stress fibers ( SFs ) 	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Lenses that translate as a whole , in shark , bony fish and frog , showed stress fibers ( SFs ) at the basal or apical end of the cells .
	manualset3
208704	6	418050	7	NULL	NULL	0	NULL	 basal end of the cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Lenses that translate as a whole , in shark , bony fish and frog , showed stress fibers ( SFs ) at the basal or apical end of the cells .
	manualset3
208705	7	418050	7	NULL	NULL	0	NULL	apical end of the cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Lenses that translate as a whole , in shark , bony fish and frog , showed stress fibers ( SFs ) at the basal or apical end of the cells .
	manualset3
208706	1	418051	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , in the dysplastic areas , there was high Ki-67 labeling index and no overexpression of p53 protein .
	manualset3
208707	2	418051	7	NULL	NULL	0	NULL	dysplastic areas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , in the dysplastic areas , there was high Ki-67 labeling index and no overexpression of p53 protein .
	manualset3
208708	3	418051	7	NULL	NULL	0	NULL	high Ki-67 labeling index	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , in the dysplastic areas , there was high Ki-67 labeling index and no overexpression of p53 protein .
	manualset3
208709	4	418051	7	NULL	NULL	0	NULL	no overexpression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , in the dysplastic areas , there was high Ki-67 labeling index and no overexpression of p53 protein .
	manualset3
208710	5	418051	7	NULL	NULL	0	NULL	p53 protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , in the dysplastic areas , there was high Ki-67 labeling index and no overexpression of p53 protein .
	manualset3
208711	1	418052	7	NULL	NULL	0	NULL	outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Use and outcomes of emergent laparoscopic resection for acute diverticulitis .
	manualset3
208712	2	418052	7	NULL	NULL	0	NULL	emergent laparoscopic resection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Use and outcomes of emergent laparoscopic resection for acute diverticulitis .
	manualset3
208713	3	418052	7	NULL	NULL	0	NULL	acute diverticulitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Use and outcomes of emergent laparoscopic resection for acute diverticulitis .
	manualset3
208714	1	418053	7	NULL	NULL	0	NULL	Antibiotic-induced bacterial cell lysis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic-induced bacterial cell lysis : a therapeutic dilemma .
	manualset3
208715	2	418053	7	NULL	NULL	0	NULL	therapeutic dilemma 	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic-induced bacterial cell lysis : a therapeutic dilemma .
	manualset3
208777	1	418054	7	NULL	NULL	0	NULL	DNA content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	I. DNA content of foetal kidneys and heart .
	manualset3
208778	2	418054	7	NULL	NULL	0	NULL	foetal kidneys	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	I. DNA content of foetal kidneys and heart .
	manualset3
208779	3	418054	7	NULL	NULL	0	NULL	heart	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	I. DNA content of foetal kidneys and heart .
	manualset3
208780	1	418055	7	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In water , the products arise through oxidation of alkyl side chains to aldehydes and carboxylic acids or through an opening in one of the aromatic rings .
	manualset3
208781	2	418055	7	NULL	NULL	0	NULL	  products	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In water , the products arise through oxidation of alkyl side chains to aldehydes and carboxylic acids or through an opening in one of the aromatic rings .
	manualset3
208782	3	418055	7	NULL	NULL	0	NULL	 oxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In water , the products arise through oxidation of alkyl side chains to aldehydes and carboxylic acids or through an opening in one of the aromatic rings .
	manualset3
208783	4	418055	7	NULL	NULL	0	NULL	alkyl side chains	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In water , the products arise through oxidation of alkyl side chains to aldehydes and carboxylic acids or through an opening in one of the aromatic rings .
	manualset3
208784	5	418055	7	NULL	NULL	0	NULL	 aldehydes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In water , the products arise through oxidation of alkyl side chains to aldehydes and carboxylic acids or through an opening in one of the aromatic rings .
	manualset3
208785	6	418055	7	NULL	NULL	0	NULL	carboxylic acids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In water , the products arise through oxidation of alkyl side chains to aldehydes and carboxylic acids or through an opening in one of the aromatic rings .
	manualset3
208786	7	418055	7	NULL	NULL	0	NULL	 opening 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In water , the products arise through oxidation of alkyl side chains to aldehydes and carboxylic acids or through an opening in one of the aromatic rings .
	manualset3
208787	8	418055	7	NULL	NULL	0	NULL	aromatic rings	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In water , the products arise through oxidation of alkyl side chains to aldehydes and carboxylic acids or through an opening in one of the aromatic rings .
	manualset3
209817	9	418055	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In water , the products arise through oxidation of alkyl side chains to aldehydes and carboxylic acids or through an opening in one of the aromatic rings .
	manualset3
208788	1	418056	7	NULL	NULL	0	NULL	 transport	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The transport of IgM into bile also appeared biphasic .
	manualset3
208789	2	418056	7	NULL	NULL	0	NULL	IgM	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The transport of IgM into bile also appeared biphasic .
	manualset3
208790	3	418056	7	NULL	NULL	0	NULL	bile 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The transport of IgM into bile also appeared biphasic .
	manualset3
208791	4	418056	7	NULL	NULL	0	NULL	biphasic	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The transport of IgM into bile also appeared biphasic .
	manualset3
208792	1	418057	7	NULL	NULL	0	NULL	Mo ( VI ) reduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mo ( VI ) reduction to molybdenum blue by Serratia marcescens strain Dr. Y9 .
	manualset3
208793	2	418057	7	NULL	NULL	0	NULL	molybdenum blue	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mo ( VI ) reduction to molybdenum blue by Serratia marcescens strain Dr. Y9 .
	manualset3
208794	3	418057	7	NULL	NULL	0	NULL	Serratia marcescens strain Dr. Y9 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mo ( VI ) reduction to molybdenum blue by Serratia marcescens strain Dr. Y9 .
	manualset3
208795	1	418058	7	NULL	NULL	0	NULL	Associations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Associations between maternal nausea during pregnancy and child behavioral outcomes were investigated in a large birth cohort .
	manualset3
208796	2	418058	7	NULL	NULL	0	NULL	maternal nausea	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Associations between maternal nausea during pregnancy and child behavioral outcomes were investigated in a large birth cohort .
	manualset3
208797	3	418058	7	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Associations between maternal nausea during pregnancy and child behavioral outcomes were investigated in a large birth cohort .
	manualset3
208798	4	418058	7	NULL	NULL	0	NULL	child behavioral outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Associations between maternal nausea during pregnancy and child behavioral outcomes were investigated in a large birth cohort .
	manualset3
208799	5	418058	7	NULL	NULL	NULL	NULL	large birth cohort 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Associations between maternal nausea during pregnancy and child behavioral outcomes were investigated in a large birth cohort .
	manualset3
208800	1	418059	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These patients generally require admittance to an intensive care unit .
	manualset3
208801	2	418059	7	NULL	NULL	0	NULL	admittance	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These patients generally require admittance to an intensive care unit .
	manualset3
208802	3	418059	7	NULL	NULL	0	NULL	 intensive care unit	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	These patients generally require admittance to an intensive care unit .
	manualset3
208803	1	418060	7	NULL	NULL	0	NULL	adult animal models 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In adult animal models , cytokine-induced neutrophil chemoattractant ( CINC ) is a potent chemoattractant for neutrophils and believed to play a role in endotoxin-induced lung injury .
	manualset3
208804	2	418060	7	NULL	NULL	0	NULL	cytokine-induced neutrophil chemoattractant ( CINC ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In adult animal models , cytokine-induced neutrophil chemoattractant ( CINC ) is a potent chemoattractant for neutrophils and believed to play a role in endotoxin-induced lung injury .
	manualset3
208805	3	418060	7	NULL	NULL	0	NULL	chemoattractant 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In adult animal models , cytokine-induced neutrophil chemoattractant ( CINC ) is a potent chemoattractant for neutrophils and believed to play a role in endotoxin-induced lung injury .
	manualset3
208806	4	418060	7	NULL	NULL	0	NULL	neutrophils	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In adult animal models , cytokine-induced neutrophil chemoattractant ( CINC ) is a potent chemoattractant for neutrophils and believed to play a role in endotoxin-induced lung injury .
	manualset3
208807	5	418060	7	NULL	NULL	0	NULL	 role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In adult animal models , cytokine-induced neutrophil chemoattractant ( CINC ) is a potent chemoattractant for neutrophils and believed to play a role in endotoxin-induced lung injury .
	manualset3
208808	6	418060	7	NULL	NULL	0	NULL	endotoxin-induced lung injury 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In adult animal models , cytokine-induced neutrophil chemoattractant ( CINC ) is a potent chemoattractant for neutrophils and believed to play a role in endotoxin-induced lung injury .
	manualset3
208809	1	418061	7	NULL	NULL	0	NULL	 first principles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Based on the first principles understanding of XPS , a GO structure model containing new oxidation species epoxy pair and epoxy-hydroxy pair is proposed .
	manualset3
208810	2	418061	7	NULL	NULL	0	NULL	XPS	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Based on the first principles understanding of XPS , a GO structure model containing new oxidation species epoxy pair and epoxy-hydroxy pair is proposed .
	manualset3
208811	3	418061	7	NULL	NULL	NULL	NULL	GO structure model 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the first principles understanding of XPS , a GO structure model containing new oxidation species epoxy pair and epoxy-hydroxy pair is proposed .
	manualset3
208812	4	418061	7	NULL	NULL	0	NULL	new oxidation species epoxy pair 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Based on the first principles understanding of XPS , a GO structure model containing new oxidation species epoxy pair and epoxy-hydroxy pair is proposed .
	manualset3
208813	5	418061	7	NULL	NULL	0	NULL	epoxy-hydroxy pair	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Based on the first principles understanding of XPS , a GO structure model containing new oxidation species epoxy pair and epoxy-hydroxy pair is proposed .
	manualset3
209818	6	418061	7	NULL	NULL	0	NULL	understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Based on the first principles understanding of XPS , a GO structure model containing new oxidation species epoxy pair and epoxy-hydroxy pair is proposed .
	manualset3
208814	1	418062	7	NULL	NULL	NULL	NULL	antagonistic efficacy	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The antagonistic efficacy of these antidotes against pinacolyl methylphosphonofluoridate may be attributed to their direct antagonism at nicotinic receptor as well as reactivation of inhibited acetylcholinesterase .
	manualset3
208815	2	418062	7	NULL	NULL	0	NULL	antidotes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The antagonistic efficacy of these antidotes against pinacolyl methylphosphonofluoridate may be attributed to their direct antagonism at nicotinic receptor as well as reactivation of inhibited acetylcholinesterase .
	manualset3
208816	3	418062	7	NULL	NULL	0	NULL	pinacolyl methylphosphonofluoridate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The antagonistic efficacy of these antidotes against pinacolyl methylphosphonofluoridate may be attributed to their direct antagonism at nicotinic receptor as well as reactivation of inhibited acetylcholinesterase .
	manualset3
208817	4	418062	7	NULL	NULL	0	NULL	direct antagonism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The antagonistic efficacy of these antidotes against pinacolyl methylphosphonofluoridate may be attributed to their direct antagonism at nicotinic receptor as well as reactivation of inhibited acetylcholinesterase .
	manualset3
208818	5	418062	7	NULL	NULL	0	NULL	nicotinic receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The antagonistic efficacy of these antidotes against pinacolyl methylphosphonofluoridate may be attributed to their direct antagonism at nicotinic receptor as well as reactivation of inhibited acetylcholinesterase .
	manualset3
208819	6	418062	7	NULL	NULL	0	NULL	 reactivation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The antagonistic efficacy of these antidotes against pinacolyl methylphosphonofluoridate may be attributed to their direct antagonism at nicotinic receptor as well as reactivation of inhibited acetylcholinesterase .
	manualset3
208820	7	418062	7	NULL	NULL	0	NULL	inhibited acetylcholinesterase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The antagonistic efficacy of these antidotes against pinacolyl methylphosphonofluoridate may be attributed to their direct antagonism at nicotinic receptor as well as reactivation of inhibited acetylcholinesterase .
	manualset3
208821	1	418063	7	NULL	NULL	0	NULL	Monday/Friday ratios	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Monday/Friday ratios were close to 1.0 , suggesting that there is no increase in melatonin production over the weekend .
	manualset3
208822	2	418063	7	NULL	NULL	0	NULL	1.0	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Monday/Friday ratios were close to 1.0 , suggesting that there is no increase in melatonin production over the weekend .
	manualset3
208823	3	418063	7	NULL	NULL	0	NULL	no increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Monday/Friday ratios were close to 1.0 , suggesting that there is no increase in melatonin production over the weekend .
	manualset3
208824	4	418063	7	NULL	NULL	0	NULL	melatonin production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Monday/Friday ratios were close to 1.0 , suggesting that there is no increase in melatonin production over the weekend .
	manualset3
208825	5	418063	7	NULL	NULL	0	NULL	weekend 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The Monday/Friday ratios were close to 1.0 , suggesting that there is no increase in melatonin production over the weekend .
	manualset3
208826	1	418064	7	NULL	NULL	NULL	NULL	ablation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Both ablation and defibrillator implantation can be shown to be cost effective in selected populations , but a cost-conscious approach to procedures and patient selection can make them cost effective in a broad range of patients .
	manualset3
208827	2	418064	7	NULL	NULL	0	NULL	 defibrillator implantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Both ablation and defibrillator implantation can be shown to be cost effective in selected populations , but a cost-conscious approach to procedures and patient selection can make them cost effective in a broad range of patients .
	manualset3
208828	3	418064	7	NULL	NULL	0	NULL	selected populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Both ablation and defibrillator implantation can be shown to be cost effective in selected populations , but a cost-conscious approach to procedures and patient selection can make them cost effective in a broad range of patients .
	manualset3
208829	4	418064	7	NULL	NULL	0	NULL	cost-conscious approach	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Both ablation and defibrillator implantation can be shown to be cost effective in selected populations , but a cost-conscious approach to procedures and patient selection can make them cost effective in a broad range of patients .
	manualset3
208830	5	418064	7	NULL	NULL	0	NULL	procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Both ablation and defibrillator implantation can be shown to be cost effective in selected populations , but a cost-conscious approach to procedures and patient selection can make them cost effective in a broad range of patients .
	manualset3
208831	6	418064	7	NULL	NULL	0	NULL	patient selection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Both ablation and defibrillator implantation can be shown to be cost effective in selected populations , but a cost-conscious approach to procedures and patient selection can make them cost effective in a broad range of patients .
	manualset3
208833	8	418064	7	NULL	NULL	0	NULL	broad range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Both ablation and defibrillator implantation can be shown to be cost effective in selected populations , but a cost-conscious approach to procedures and patient selection can make them cost effective in a broad range of patients .
	manualset3
208834	9	418064	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Both ablation and defibrillator implantation can be shown to be cost effective in selected populations , but a cost-conscious approach to procedures and patient selection can make them cost effective in a broad range of patients .
	manualset3
208835	1	418065	7	NULL	NULL	NULL	NULL	Errors	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Errors are viewed , in nonlinear dynamical terms , as brief-duration changes in stationary presynaptic spike trains which induce transient responses in the postsynaptic cell .
	manualset3
208836	2	418065	7	NULL	NULL	NULL	NULL	nonlinear dynamical terms	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Errors are viewed , in nonlinear dynamical terms , as brief-duration changes in stationary presynaptic spike trains which induce transient responses in the postsynaptic cell .
	manualset3
208837	3	418065	7	NULL	NULL	0	NULL	brief-duration changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Errors are viewed , in nonlinear dynamical terms , as brief-duration changes in stationary presynaptic spike trains which induce transient responses in the postsynaptic cell .
	manualset3
208838	4	418065	7	NULL	NULL	0	NULL	stationary presynaptic spike trains 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Errors are viewed , in nonlinear dynamical terms , as brief-duration changes in stationary presynaptic spike trains which induce transient responses in the postsynaptic cell .
	manualset3
208839	5	418065	7	NULL	NULL	0	NULL	transient responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Errors are viewed , in nonlinear dynamical terms , as brief-duration changes in stationary presynaptic spike trains which induce transient responses in the postsynaptic cell .
	manualset3
208840	6	418065	7	NULL	NULL	0	NULL	postsynaptic cell 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Errors are viewed , in nonlinear dynamical terms , as brief-duration changes in stationary presynaptic spike trains which induce transient responses in the postsynaptic cell .
	manualset3
208841	1	418066	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , among children aged 59 months requiring additional primary series doses , PCV13 coverage was only 46 % .
	manualset3
208842	2	418066	7	NULL	NULL	NULL	NULL	59 months	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Similarly , among children aged 59 months requiring additional primary series doses , PCV13 coverage was only 46 % .
	manualset3
208843	3	418066	7	NULL	NULL	0	NULL	primary series doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , among children aged 59 months requiring additional primary series doses , PCV13 coverage was only 46 % .
	manualset3
208844	4	418066	7	NULL	NULL	0	NULL	 PCV13 coverage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , among children aged 59 months requiring additional primary series doses , PCV13 coverage was only 46 % .
	manualset3
208845	5	418066	7	NULL	NULL	0	NULL	46 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , among children aged 59 months requiring additional primary series doses , PCV13 coverage was only 46 % .
	manualset3
208846	1	418067	7	NULL	NULL	0	NULL	Cyclophosphamide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Cyclophosphamide , vincristine , and prednisone ( CVP ) versus adriamycin , bleomycin , and prednisone ( ABP ) in stage IV non-Hodgkin 's lymphomas .
	manualset3
208847	2	418067	7	NULL	NULL	0	NULL	 vincristine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Cyclophosphamide , vincristine , and prednisone ( CVP ) versus adriamycin , bleomycin , and prednisone ( ABP ) in stage IV non-Hodgkin 's lymphomas .
	manualset3
208848	3	418067	7	NULL	NULL	0	NULL	prednisone ( CVP )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Cyclophosphamide , vincristine , and prednisone ( CVP ) versus adriamycin , bleomycin , and prednisone ( ABP ) in stage IV non-Hodgkin 's lymphomas .
	manualset3
208849	4	418067	7	NULL	NULL	0	NULL	adriamycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Cyclophosphamide , vincristine , and prednisone ( CVP ) versus adriamycin , bleomycin , and prednisone ( ABP ) in stage IV non-Hodgkin 's lymphomas .
	manualset3
208850	5	418067	7	NULL	NULL	0	NULL	 bleomycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Cyclophosphamide , vincristine , and prednisone ( CVP ) versus adriamycin , bleomycin , and prednisone ( ABP ) in stage IV non-Hodgkin 's lymphomas .
	manualset3
208851	6	418067	7	NULL	NULL	0	NULL	prednisone ( ABP )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Cyclophosphamide , vincristine , and prednisone ( CVP ) versus adriamycin , bleomycin , and prednisone ( ABP ) in stage IV non-Hodgkin 's lymphomas .
	manualset3
208852	7	418067	7	NULL	NULL	0	NULL	stage IV non-Hodgkin 's lymphomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Cyclophosphamide , vincristine , and prednisone ( CVP ) versus adriamycin , bleomycin , and prednisone ( ABP ) in stage IV non-Hodgkin 's lymphomas .
	manualset3
208853	1	418068	7	NULL	NULL	0	NULL	Serum thymidine kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum thymidine kinase in transplant patients : its relation to cytomegalovirus activity , renal transplant rejection and its use for monitoring of antiviral therapy .
	manualset3
208854	2	418068	7	NULL	NULL	0	NULL	transplant patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum thymidine kinase in transplant patients : its relation to cytomegalovirus activity , renal transplant rejection and its use for monitoring of antiviral therapy .
	manualset3
208855	3	418068	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum thymidine kinase in transplant patients : its relation to cytomegalovirus activity , renal transplant rejection and its use for monitoring of antiviral therapy .
	manualset3
208856	4	418068	7	NULL	NULL	0	NULL	cytomegalovirus activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum thymidine kinase in transplant patients : its relation to cytomegalovirus activity , renal transplant rejection and its use for monitoring of antiviral therapy .
	manualset3
208857	5	418068	7	NULL	NULL	0	NULL	renal transplant rejection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum thymidine kinase in transplant patients : its relation to cytomegalovirus activity , renal transplant rejection and its use for monitoring of antiviral therapy .
	manualset3
208858	6	418068	7	NULL	NULL	0	NULL	monitoring	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum thymidine kinase in transplant patients : its relation to cytomegalovirus activity , renal transplant rejection and its use for monitoring of antiviral therapy .
	manualset3
208859	7	418068	7	NULL	NULL	0	NULL	antiviral therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum thymidine kinase in transplant patients : its relation to cytomegalovirus activity , renal transplant rejection and its use for monitoring of antiviral therapy .
	manualset3
208860	1	418069	7	NULL	NULL	0	NULL	studied factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	All the studied factors were significantly associated with the treatment need for TMD at all examinations .
	manualset3
208861	2	418069	7	NULL	NULL	0	NULL	 treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All the studied factors were significantly associated with the treatment need for TMD at all examinations .
	manualset3
208862	3	418069	7	NULL	NULL	0	NULL	TMD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	All the studied factors were significantly associated with the treatment need for TMD at all examinations .
	manualset3
208863	4	418069	7	NULL	NULL	0	NULL	examinations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All the studied factors were significantly associated with the treatment need for TMD at all examinations .
	manualset3
208864	1	418070	7	NULL	NULL	0	NULL	availability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Despite the availability of low-molecular-weight heparins , unfractionated heparin ( UFH ) still remains the drug of choice for the initial treatment of acute venous thromboembolism in many countries .
	manualset3
208865	2	418070	7	NULL	NULL	0	NULL	low-molecular-weight heparins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Despite the availability of low-molecular-weight heparins , unfractionated heparin ( UFH ) still remains the drug of choice for the initial treatment of acute venous thromboembolism in many countries .
	manualset3
208866	3	418070	7	NULL	NULL	0	NULL	unfractionated heparin ( UFH )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Despite the availability of low-molecular-weight heparins , unfractionated heparin ( UFH ) still remains the drug of choice for the initial treatment of acute venous thromboembolism in many countries .
	manualset3
208867	4	418070	7	NULL	NULL	0	NULL	drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Despite the availability of low-molecular-weight heparins , unfractionated heparin ( UFH ) still remains the drug of choice for the initial treatment of acute venous thromboembolism in many countries .
	manualset3
208868	5	418070	7	NULL	NULL	0	NULL	 initial treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Despite the availability of low-molecular-weight heparins , unfractionated heparin ( UFH ) still remains the drug of choice for the initial treatment of acute venous thromboembolism in many countries .
	manualset3
208869	6	418070	7	NULL	NULL	0	NULL	acute venous thromboembolism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Despite the availability of low-molecular-weight heparins , unfractionated heparin ( UFH ) still remains the drug of choice for the initial treatment of acute venous thromboembolism in many countries .
	manualset3
208870	7	418070	7	NULL	NULL	0	NULL	countries	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Despite the availability of low-molecular-weight heparins , unfractionated heparin ( UFH ) still remains the drug of choice for the initial treatment of acute venous thromboembolism in many countries .
	manualset3
208871	1	418071	7	NULL	NULL	0	NULL	fluoroquinolones	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Newer fluoroquinolones with increased in vitro activity against anaerobes are under development and include levofloxacin , clinafloxacin , sparfloxacin , trovafloxacin , grepafloxacin , and DU-6859a .
	manualset3
208872	2	418071	7	NULL	NULL	0	NULL	increased in vitro activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Newer fluoroquinolones with increased in vitro activity against anaerobes are under development and include levofloxacin , clinafloxacin , sparfloxacin , trovafloxacin , grepafloxacin , and DU-6859a .
	manualset3
208873	3	418071	7	NULL	NULL	0	NULL	anaerobes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Newer fluoroquinolones with increased in vitro activity against anaerobes are under development and include levofloxacin , clinafloxacin , sparfloxacin , trovafloxacin , grepafloxacin , and DU-6859a .
	manualset3
208874	4	418071	7	NULL	NULL	0	NULL	 levofloxacin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Newer fluoroquinolones with increased in vitro activity against anaerobes are under development and include levofloxacin , clinafloxacin , sparfloxacin , trovafloxacin , grepafloxacin , and DU-6859a .
	manualset3
208875	5	418071	7	NULL	NULL	0	NULL	clinafloxacin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Newer fluoroquinolones with increased in vitro activity against anaerobes are under development and include levofloxacin , clinafloxacin , sparfloxacin , trovafloxacin , grepafloxacin , and DU-6859a .
	manualset3
208876	6	418071	7	NULL	NULL	0	NULL	 sparfloxacin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Newer fluoroquinolones with increased in vitro activity against anaerobes are under development and include levofloxacin , clinafloxacin , sparfloxacin , trovafloxacin , grepafloxacin , and DU-6859a .
	manualset3
208877	7	418071	7	NULL	NULL	0	NULL	trovafloxacin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Newer fluoroquinolones with increased in vitro activity against anaerobes are under development and include levofloxacin , clinafloxacin , sparfloxacin , trovafloxacin , grepafloxacin , and DU-6859a .
	manualset3
208878	8	418071	7	NULL	NULL	0	NULL	grepafloxacin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Newer fluoroquinolones with increased in vitro activity against anaerobes are under development and include levofloxacin , clinafloxacin , sparfloxacin , trovafloxacin , grepafloxacin , and DU-6859a .
	manualset3
208879	9	418071	7	NULL	NULL	0	NULL	DU-6859a	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Newer fluoroquinolones with increased in vitro activity against anaerobes are under development and include levofloxacin , clinafloxacin , sparfloxacin , trovafloxacin , grepafloxacin , and DU-6859a .
	manualset3
208880	10	418071	7	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Newer fluoroquinolones with increased in vitro activity against anaerobes are under development and include levofloxacin , clinafloxacin , sparfloxacin , trovafloxacin , grepafloxacin , and DU-6859a .
	manualset3
208881	1	418072	7	NULL	NULL	0	NULL	Background	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Background The rise in non-communicable diseases in developing countries has gained increased attention .
	manualset3
208882	2	418072	7	NULL	NULL	0	NULL	rise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Background The rise in non-communicable diseases in developing countries has gained increased attention .
	manualset3
208883	3	418072	7	NULL	NULL	0	NULL	non-communicable diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Background The rise in non-communicable diseases in developing countries has gained increased attention .
	manualset3
208884	4	418072	7	NULL	NULL	0	NULL	developing countries	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Background The rise in non-communicable diseases in developing countries has gained increased attention .
	manualset3
208885	5	418072	7	NULL	NULL	0	NULL	increased attention	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Background The rise in non-communicable diseases in developing countries has gained increased attention .
	manualset3
208886	1	418073	7	NULL	NULL	0	NULL	Prophylactic oophorectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prophylactic oophorectomy has been recommended in patients with a strongly positive family history for ovarian carcinoma .
	manualset3
208887	2	418073	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Prophylactic oophorectomy has been recommended in patients with a strongly positive family history for ovarian carcinoma .
	manualset3
208888	3	418073	7	NULL	NULL	0	NULL	 strongly positive family history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prophylactic oophorectomy has been recommended in patients with a strongly positive family history for ovarian carcinoma .
	manualset3
208889	4	418073	7	NULL	NULL	0	NULL	 ovarian carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Prophylactic oophorectomy has been recommended in patients with a strongly positive family history for ovarian carcinoma .
	manualset3
208890	1	418074	7	NULL	NULL	0	NULL	muscarinic toxins	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The muscarinic toxins appear to be invaluable tools to study receptor pharmacology , physiology and structure/function relationships .
	manualset3
208891	2	418074	7	NULL	NULL	0	NULL	 invaluable tools	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The muscarinic toxins appear to be invaluable tools to study receptor pharmacology , physiology and structure/function relationships .
	manualset3
208892	3	418074	7	NULL	NULL	0	NULL	 receptor pharmacology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The muscarinic toxins appear to be invaluable tools to study receptor pharmacology , physiology and structure/function relationships .
	manualset3
208893	4	418074	7	NULL	NULL	0	NULL	physiology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The muscarinic toxins appear to be invaluable tools to study receptor pharmacology , physiology and structure/function relationships .
	manualset3
208894	5	418074	7	NULL	NULL	0	NULL	structure/function relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The muscarinic toxins appear to be invaluable tools to study receptor pharmacology , physiology and structure/function relationships .
	manualset3
208895	1	418075	7	NULL	NULL	0	NULL	 use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of alkaline media presents advantages both in electrocatalytic activity and in materials stability and corrosion .
	manualset3
208896	2	418075	7	NULL	NULL	0	NULL	alkaline media 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of alkaline media presents advantages both in electrocatalytic activity and in materials stability and corrosion .
	manualset3
208897	3	418075	7	NULL	NULL	0	NULL	electrocatalytic activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of alkaline media presents advantages both in electrocatalytic activity and in materials stability and corrosion .
	manualset3
208898	4	418075	7	NULL	NULL	0	NULL	materials stability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of alkaline media presents advantages both in electrocatalytic activity and in materials stability and corrosion .
	manualset3
208899	5	418075	7	NULL	NULL	0	NULL	corrosion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of alkaline media presents advantages both in electrocatalytic activity and in materials stability and corrosion .
	manualset3
208900	1	418076	7	NULL	NULL	0	NULL	Psychologists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychologists are encouraged to investigate the psychopathy-treatment relation from multiple perspectives as well as to conduct long-term follow-up studies to establish a modern view of the psychopathy-treatment relation .
	manualset3
208901	2	418076	7	NULL	NULL	0	NULL	psychopathy-treatment relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychologists are encouraged to investigate the psychopathy-treatment relation from multiple perspectives as well as to conduct long-term follow-up studies to establish a modern view of the psychopathy-treatment relation .
	manualset3
208902	3	418076	7	NULL	NULL	0	NULL	multiple perspectives	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychologists are encouraged to investigate the psychopathy-treatment relation from multiple perspectives as well as to conduct long-term follow-up studies to establish a modern view of the psychopathy-treatment relation .
	manualset3
208903	4	418076	7	NULL	NULL	0	NULL	long-term follow-up studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychologists are encouraged to investigate the psychopathy-treatment relation from multiple perspectives as well as to conduct long-term follow-up studies to establish a modern view of the psychopathy-treatment relation .
	manualset3
208904	5	418076	7	NULL	NULL	NULL	NULL	modern view	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Psychologists are encouraged to investigate the psychopathy-treatment relation from multiple perspectives as well as to conduct long-term follow-up studies to establish a modern view of the psychopathy-treatment relation .
	manualset3
208905	6	418076	7	NULL	NULL	0	NULL	psychopathy-treatment relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Psychologists are encouraged to investigate the psychopathy-treatment relation from multiple perspectives as well as to conduct long-term follow-up studies to establish a modern view of the psychopathy-treatment relation .
	manualset3
208906	1	418077	7	NULL	NULL	0	NULL	FGF23 neutralization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	FGF23 neutralization improves chronic kidney disease-associated hyperparathyroidism yet increases mortality .
	manualset3
208907	2	418077	7	NULL	NULL	0	NULL	 chronic kidney disease-associated hyperparathyroidism	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	FGF23 neutralization improves chronic kidney disease-associated hyperparathyroidism yet increases mortality .
	manualset3
208908	3	418077	7	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	FGF23 neutralization improves chronic kidney disease-associated hyperparathyroidism yet increases mortality .
	manualset3
208909	1	418078	7	NULL	NULL	0	NULL	subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All the subjects were studied with inhalation challenges with TDI and with methacholine .
	manualset3
208910	2	418078	7	NULL	NULL	0	NULL	inhalation challenges	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All the subjects were studied with inhalation challenges with TDI and with methacholine .
	manualset3
208911	3	418078	7	NULL	NULL	0	NULL	TDI	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All the subjects were studied with inhalation challenges with TDI and with methacholine .
	manualset3
208912	4	418078	7	NULL	NULL	0	NULL	methacholine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All the subjects were studied with inhalation challenges with TDI and with methacholine .
	manualset3
208913	1	418079	7	NULL	NULL	0	NULL	Ocular manifestations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ocular manifestations of systemic diseases .
	manualset3
208914	2	418079	7	NULL	NULL	0	NULL	systemic diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Ocular manifestations of systemic diseases .
	manualset3
208915	1	418080	7	NULL	NULL	0	NULL	 childhood mortalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The childhood & infant mortalities have reduced to less than half , but after an initial fall there was very little further improvement in perinatal and neonatal mortality .
	manualset3
208916	2	418080	7	NULL	NULL	0	NULL	infant mortalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The childhood & infant mortalities have reduced to less than half , but after an initial fall there was very little further improvement in perinatal and neonatal mortality .
	manualset3
208917	3	418080	7	NULL	NULL	0	NULL	 initial fall 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The childhood & infant mortalities have reduced to less than half , but after an initial fall there was very little further improvement in perinatal and neonatal mortality .
	manualset3
208918	4	418080	7	NULL	NULL	0	NULL	 improvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The childhood & infant mortalities have reduced to less than half , but after an initial fall there was very little further improvement in perinatal and neonatal mortality .
	manualset3
208919	5	418080	7	NULL	NULL	0	NULL	perinatal mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The childhood & infant mortalities have reduced to less than half , but after an initial fall there was very little further improvement in perinatal and neonatal mortality .
	manualset3
208920	6	418080	7	NULL	NULL	0	NULL	neonatal mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The childhood & infant mortalities have reduced to less than half , but after an initial fall there was very little further improvement in perinatal and neonatal mortality .
	manualset3
208921	1	418081	7	NULL	NULL	0	NULL	garden dormouse protein deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In garden dormouse protein deficiency leads to reversible hypothermic torpor , comparable with that provoked by starvation or occuring naturally during hibernation , whether the diet consists wholly of apples or of synthetic protein-free food .
	manualset3
208922	2	418081	7	NULL	NULL	0	NULL	reversible hypothermic torpor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In garden dormouse protein deficiency leads to reversible hypothermic torpor , comparable with that provoked by starvation or occuring naturally during hibernation , whether the diet consists wholly of apples or of synthetic protein-free food .
	manualset3
208923	3	418081	7	NULL	NULL	0	NULL	starvation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In garden dormouse protein deficiency leads to reversible hypothermic torpor , comparable with that provoked by starvation or occuring naturally during hibernation , whether the diet consists wholly of apples or of synthetic protein-free food .
	manualset3
208924	4	418081	7	NULL	NULL	0	NULL	hibernation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In garden dormouse protein deficiency leads to reversible hypothermic torpor , comparable with that provoked by starvation or occuring naturally during hibernation , whether the diet consists wholly of apples or of synthetic protein-free food .
	manualset3
208925	5	418081	7	NULL	NULL	0	NULL	 diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	In garden dormouse protein deficiency leads to reversible hypothermic torpor , comparable with that provoked by starvation or occuring naturally during hibernation , whether the diet consists wholly of apples or of synthetic protein-free food .
	manualset3
208926	6	418081	7	NULL	NULL	0	NULL	apples	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	In garden dormouse protein deficiency leads to reversible hypothermic torpor , comparable with that provoked by starvation or occuring naturally during hibernation , whether the diet consists wholly of apples or of synthetic protein-free food .
	manualset3
208927	7	418081	7	NULL	NULL	0	NULL	synthetic protein-free food	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	In garden dormouse protein deficiency leads to reversible hypothermic torpor , comparable with that provoked by starvation or occuring naturally during hibernation , whether the diet consists wholly of apples or of synthetic protein-free food .
	manualset3
208928	1	418082	7	NULL	NULL	0	NULL	Radiolabelled immunoglobulins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiolabelled immunoglobulins were taken up by the worms and shown to localize as fine strands running perpendicular to the parasite surface .
	manualset3
208929	2	418082	7	NULL	NULL	0	NULL	worms 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiolabelled immunoglobulins were taken up by the worms and shown to localize as fine strands running perpendicular to the parasite surface .
	manualset3
208930	3	418082	7	NULL	NULL	0	NULL	fine strands	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiolabelled immunoglobulins were taken up by the worms and shown to localize as fine strands running perpendicular to the parasite surface .
	manualset3
208931	4	418082	7	NULL	NULL	0	NULL	parasite surface	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiolabelled immunoglobulins were taken up by the worms and shown to localize as fine strands running perpendicular to the parasite surface .
	manualset3
208932	1	418083	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with carbamazepine , serum doxepin and doxepin + nordoxepin concentrations ( N = 17 ) were decreased significantly ( p less than 0.05 ) , on average to 46 % and 45 % , respectively , as compared to that in subjects without carbamazepine .
	manualset3
208933	2	418083	7	NULL	NULL	0	NULL	carbamazepine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with carbamazepine , serum doxepin and doxepin + nordoxepin concentrations ( N = 17 ) were decreased significantly ( p less than 0.05 ) , on average to 46 % and 45 % , respectively , as compared to that in subjects without carbamazepine .
	manualset3
208934	3	418083	7	NULL	NULL	0	NULL	serum doxepin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with carbamazepine , serum doxepin and doxepin + nordoxepin concentrations ( N = 17 ) were decreased significantly ( p less than 0.05 ) , on average to 46 % and 45 % , respectively , as compared to that in subjects without carbamazepine .
	manualset3
208935	4	418083	7	NULL	NULL	0	NULL	doxepin + nordoxepin concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with carbamazepine , serum doxepin and doxepin + nordoxepin concentrations ( N = 17 ) were decreased significantly ( p less than 0.05 ) , on average to 46 % and 45 % , respectively , as compared to that in subjects without carbamazepine .
	manualset3
208936	5	418083	7	NULL	NULL	0	NULL	N = 17	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with carbamazepine , serum doxepin and doxepin + nordoxepin concentrations ( N = 17 ) were decreased significantly ( p less than 0.05 ) , on average to 46 % and 45 % , respectively , as compared to that in subjects without carbamazepine .
	manualset3
208937	6	418083	7	NULL	NULL	0	NULL	p less than 0.05	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with carbamazepine , serum doxepin and doxepin + nordoxepin concentrations ( N = 17 ) were decreased significantly ( p less than 0.05 ) , on average to 46 % and 45 % , respectively , as compared to that in subjects without carbamazepine .
	manualset3
208938	7	418083	7	NULL	NULL	0	NULL	46 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with carbamazepine , serum doxepin and doxepin + nordoxepin concentrations ( N = 17 ) were decreased significantly ( p less than 0.05 ) , on average to 46 % and 45 % , respectively , as compared to that in subjects without carbamazepine .
	manualset3
208939	8	418083	7	NULL	NULL	0	NULL	45 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with carbamazepine , serum doxepin and doxepin + nordoxepin concentrations ( N = 17 ) were decreased significantly ( p less than 0.05 ) , on average to 46 % and 45 % , respectively , as compared to that in subjects without carbamazepine .
	manualset3
208940	9	418083	7	NULL	NULL	0	NULL	subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with carbamazepine , serum doxepin and doxepin + nordoxepin concentrations ( N = 17 ) were decreased significantly ( p less than 0.05 ) , on average to 46 % and 45 % , respectively , as compared to that in subjects without carbamazepine .
	manualset3
208941	10	418083	7	NULL	NULL	0	NULL	carbamazepine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with carbamazepine , serum doxepin and doxepin + nordoxepin concentrations ( N = 17 ) were decreased significantly ( p less than 0.05 ) , on average to 46 % and 45 % , respectively , as compared to that in subjects without carbamazepine .
	manualset3
208942	1	418084	7	NULL	NULL	0	NULL	 gastric acidity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , the gastric acidity is buffered , sometimes during many hours : that decreases or cancels the gastro-esophageal pH gradient .
	manualset3
208943	2	418084	7	NULL	NULL	0	NULL	hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , the gastric acidity is buffered , sometimes during many hours : that decreases or cancels the gastro-esophageal pH gradient .
	manualset3
208944	3	418084	7	NULL	NULL	0	NULL	gastro-esophageal pH gradient	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , the gastric acidity is buffered , sometimes during many hours : that decreases or cancels the gastro-esophageal pH gradient .
	manualset3
208945	1	418085	7	NULL	NULL	0	NULL	Pout/Pin ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Pout/Pin ratio was 160 + / - 78 for F and 26 + / - 9 for FG .
	manualset3
208946	2	418085	7	NULL	NULL	0	NULL	160 + / - 78 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Pout/Pin ratio was 160 + / - 78 for F and 26 + / - 9 for FG .
	manualset3
208947	3	418085	7	NULL	NULL	0	NULL	 F	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The Pout/Pin ratio was 160 + / - 78 for F and 26 + / - 9 for FG .
	manualset3
208948	4	418085	7	NULL	NULL	0	NULL	26 + / - 9	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The Pout/Pin ratio was 160 + / - 78 for F and 26 + / - 9 for FG .
	manualset3
208949	5	418085	7	NULL	NULL	0	NULL	FG	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The Pout/Pin ratio was 160 + / - 78 for F and 26 + / - 9 for FG .
	manualset3
208950	1	418086	7	NULL	NULL	NULL	NULL	Staple	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Staple versus fibrin glue fixation in laparoscopic total extraperitoneal repair of inguinal hernia : a systematic review and meta-analysis .
	manualset3
208951	2	418086	7	NULL	NULL	0	NULL	fibrin glue fixation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Staple versus fibrin glue fixation in laparoscopic total extraperitoneal repair of inguinal hernia : a systematic review and meta-analysis .
	manualset3
208952	3	418086	7	NULL	NULL	0	NULL	 laparoscopic total extraperitoneal repair	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Staple versus fibrin glue fixation in laparoscopic total extraperitoneal repair of inguinal hernia : a systematic review and meta-analysis .
	manualset3
208953	4	418086	7	NULL	NULL	NULL	NULL	inguinal hernia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Staple versus fibrin glue fixation in laparoscopic total extraperitoneal repair of inguinal hernia : a systematic review and meta-analysis .
	manualset3
208954	5	418086	7	NULL	NULL	0	NULL	systematic review 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Staple versus fibrin glue fixation in laparoscopic total extraperitoneal repair of inguinal hernia : a systematic review and meta-analysis .
	manualset3
208955	6	418086	7	NULL	NULL	0	NULL	meta-analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Staple versus fibrin glue fixation in laparoscopic total extraperitoneal repair of inguinal hernia : a systematic review and meta-analysis .
	manualset3
208956	1	418087	7	NULL	NULL	NULL	NULL	ages 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the ages of 24 and 36 months , boys were more aggressive than girls .
	manualset3
208957	2	418087	7	NULL	NULL	0	NULL	24 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	At the ages of 24 and 36 months , boys were more aggressive than girls .
	manualset3
208958	3	418087	7	NULL	NULL	0	NULL	 36 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	At the ages of 24 and 36 months , boys were more aggressive than girls .
	manualset3
208959	4	418087	7	NULL	NULL	0	NULL	boys	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	At the ages of 24 and 36 months , boys were more aggressive than girls .
	manualset3
208960	5	418087	7	NULL	NULL	0	NULL	girls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	At the ages of 24 and 36 months , boys were more aggressive than girls .
	manualset3
208961	6	418087	7	NULL	NULL	0	NULL	aggressive	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	At the ages of 24 and 36 months , boys were more aggressive than girls .
	manualset3
208962	1	418088	7	NULL	NULL	0	NULL	metformin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	We show here that metformin acts as a growth inhibitor rather than an insulin sensitizer for epithelial cells .
	manualset3
208963	2	418088	7	NULL	NULL	0	NULL	growth inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We show here that metformin acts as a growth inhibitor rather than an insulin sensitizer for epithelial cells .
	manualset3
208964	3	418088	7	NULL	NULL	0	NULL	insulin sensitizer 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We show here that metformin acts as a growth inhibitor rather than an insulin sensitizer for epithelial cells .
	manualset3
208965	4	418088	7	NULL	NULL	0	NULL	epithelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We show here that metformin acts as a growth inhibitor rather than an insulin sensitizer for epithelial cells .
	manualset3
208966	1	418089	7	NULL	NULL	0	NULL	synthesized compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All the synthesized compounds were evaluated for cytotoxic activity against two human monocytic cell lines ( U 937 , THP-1 ) and a mouse melanoma cell line ( B16-F10 ) .
	manualset3
208967	2	418089	7	NULL	NULL	0	NULL	cytotoxic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All the synthesized compounds were evaluated for cytotoxic activity against two human monocytic cell lines ( U 937 , THP-1 ) and a mouse melanoma cell line ( B16-F10 ) .
	manualset3
208968	3	418089	7	NULL	NULL	0	NULL	two human monocytic cell lines (	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	All the synthesized compounds were evaluated for cytotoxic activity against two human monocytic cell lines ( U 937 , THP-1 ) and a mouse melanoma cell line ( B16-F10 ) .
	manualset3
208969	4	418089	7	NULL	NULL	0	NULL	U 937	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	All the synthesized compounds were evaluated for cytotoxic activity against two human monocytic cell lines ( U 937 , THP-1 ) and a mouse melanoma cell line ( B16-F10 ) .
	manualset3
208970	5	418089	7	NULL	NULL	0	NULL	THP-1	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	All the synthesized compounds were evaluated for cytotoxic activity against two human monocytic cell lines ( U 937 , THP-1 ) and a mouse melanoma cell line ( B16-F10 ) .
	manualset3
208971	6	418089	7	NULL	NULL	0	NULL	 mouse melanoma cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	All the synthesized compounds were evaluated for cytotoxic activity against two human monocytic cell lines ( U 937 , THP-1 ) and a mouse melanoma cell line ( B16-F10 ) .
	manualset3
208972	7	418089	7	NULL	NULL	0	NULL	B16-F10	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	All the synthesized compounds were evaluated for cytotoxic activity against two human monocytic cell lines ( U 937 , THP-1 ) and a mouse melanoma cell line ( B16-F10 ) .
	manualset3
208973	1	418090	7	NULL	NULL	0	NULL	Contemporary gene flow	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contemporary gene flow was not severely limited for A. sapidus as shown by high migration rates estimates ( & gt ; 10 % ) between non-neighbouring areas .
	manualset3
208974	2	418090	7	NULL	NULL	0	NULL	A. sapidus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Contemporary gene flow was not severely limited for A. sapidus as shown by high migration rates estimates ( & gt ; 10 % ) between non-neighbouring areas .
	manualset3
208975	3	418090	7	NULL	NULL	0	NULL	 high migration rates estimates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Contemporary gene flow was not severely limited for A. sapidus as shown by high migration rates estimates ( & gt ; 10 % ) between non-neighbouring areas .
	manualset3
208976	4	418090	7	NULL	NULL	0	NULL	& gt ; 10 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Contemporary gene flow was not severely limited for A. sapidus as shown by high migration rates estimates ( & gt ; 10 % ) between non-neighbouring areas .
	manualset3
208977	5	418090	7	NULL	NULL	0	NULL	non-neighbouring areas	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Contemporary gene flow was not severely limited for A. sapidus as shown by high migration rates estimates ( & gt ; 10 % ) between non-neighbouring areas .
	manualset3
208978	1	418091	7	NULL	NULL	0	NULL	Golgi association	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Golgi association and the bipartite structure along with the differential targeting of its domains suggest that Vear is involved in heterotypic vesicle/suborganelle interactions associated with the Golgi complex .
	manualset3
208979	2	418091	7	NULL	NULL	0	NULL	bipartite structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Golgi association and the bipartite structure along with the differential targeting of its domains suggest that Vear is involved in heterotypic vesicle/suborganelle interactions associated with the Golgi complex .
	manualset3
208980	3	418091	7	NULL	NULL	0	NULL	differential targeting	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Golgi association and the bipartite structure along with the differential targeting of its domains suggest that Vear is involved in heterotypic vesicle/suborganelle interactions associated with the Golgi complex .
	manualset3
208981	4	418091	7	NULL	NULL	0	NULL	 domains	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The Golgi association and the bipartite structure along with the differential targeting of its domains suggest that Vear is involved in heterotypic vesicle/suborganelle interactions associated with the Golgi complex .
	manualset3
208982	5	418091	7	NULL	NULL	0	NULL	 Vear	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The Golgi association and the bipartite structure along with the differential targeting of its domains suggest that Vear is involved in heterotypic vesicle/suborganelle interactions associated with the Golgi complex .
	manualset3
208983	6	418091	7	NULL	NULL	0	NULL	heterotypic vesicle/suborganelle interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Golgi association and the bipartite structure along with the differential targeting of its domains suggest that Vear is involved in heterotypic vesicle/suborganelle interactions associated with the Golgi complex .
	manualset3
208984	7	418091	7	NULL	NULL	0	NULL	Golgi complex	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The Golgi association and the bipartite structure along with the differential targeting of its domains suggest that Vear is involved in heterotypic vesicle/suborganelle interactions associated with the Golgi complex .
	manualset3
208985	1	418092	7	NULL	NULL	0	NULL	response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The response of PRL to TRH stimulation was exaggerated in 2 , normal in 6 and absent in 2 patients .
	manualset3
208986	2	418092	7	NULL	NULL	0	NULL	PRL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The response of PRL to TRH stimulation was exaggerated in 2 , normal in 6 and absent in 2 patients .
	manualset3
208987	3	418092	7	NULL	NULL	NULL	NULL	TRH stimulation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The response of PRL to TRH stimulation was exaggerated in 2 , normal in 6 and absent in 2 patients .
	manualset3
208988	4	418092	7	NULL	NULL	NULL	NULL	2 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The response of PRL to TRH stimulation was exaggerated in 2 , normal in 6 and absent in 2 patients .
	manualset3
208989	5	418092	7	NULL	NULL	NULL	NULL	6 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The response of PRL to TRH stimulation was exaggerated in 2 , normal in 6 and absent in 2 patients .
	manualset3
208990	6	418092	7	NULL	NULL	NULL	NULL	2 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The response of PRL to TRH stimulation was exaggerated in 2 , normal in 6 and absent in 2 patients .
	manualset3
208992	1	418093	7	NULL	NULL	0	NULL	improved calculations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , our new improved calculations support for the proposed His291 model of the CcO pump .
	manualset3
208993	2	418093	7	NULL	NULL	0	NULL	His291 model 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , our new improved calculations support for the proposed His291 model of the CcO pump .
	manualset3
208994	3	418093	7	NULL	NULL	0	NULL	CcO pump	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , our new improved calculations support for the proposed His291 model of the CcO pump .
	manualset3
208995	1	418094	7	NULL	NULL	0	NULL	reconstituted lipoprotein assembly	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We have reconstituted lipoprotein assembly in an insect cell line that normally does not support this process .
	manualset3
208996	2	418094	7	NULL	NULL	0	NULL	insect cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We have reconstituted lipoprotein assembly in an insect cell line that normally does not support this process .
	manualset3
208997	3	418094	7	NULL	NULL	0	NULL	 process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We have reconstituted lipoprotein assembly in an insect cell line that normally does not support this process .
	manualset3
208998	1	418095	7	NULL	NULL	0	NULL	monotonic decrease 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We found a monotonic decrease in mean cycle length with increasing total THM ( TTHM ) level ; at ) 60 microg/L , the adjusted decrement was 1.1 days ( 95 % confidence interval ( CI ) , -1.8 to -0.40 ) , compared with less than or equal to 40 microg/L .
	manualset3
208999	2	418095	7	NULL	NULL	0	NULL	mean cycle length	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We found a monotonic decrease in mean cycle length with increasing total THM ( TTHM ) level ; at ) 60 microg/L , the adjusted decrement was 1.1 days ( 95 % confidence interval ( CI ) , -1.8 to -0.40 ) , compared with less than or equal to 40 microg/L .
	manualset3
209000	3	418095	7	NULL	NULL	0	NULL	increasing total THM ( TTHM ) level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We found a monotonic decrease in mean cycle length with increasing total THM ( TTHM ) level ; at ) 60 microg/L , the adjusted decrement was 1.1 days ( 95 % confidence interval ( CI ) , -1.8 to -0.40 ) , compared with less than or equal to 40 microg/L .
	manualset3
209001	4	418095	7	NULL	NULL	0	NULL	60 microg/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	We found a monotonic decrease in mean cycle length with increasing total THM ( TTHM ) level ; at ) 60 microg/L , the adjusted decrement was 1.1 days ( 95 % confidence interval ( CI ) , -1.8 to -0.40 ) , compared with less than or equal to 40 microg/L .
	manualset3
209002	5	418095	7	NULL	NULL	0	NULL	decrement	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We found a monotonic decrease in mean cycle length with increasing total THM ( TTHM ) level ; at ) 60 microg/L , the adjusted decrement was 1.1 days ( 95 % confidence interval ( CI ) , -1.8 to -0.40 ) , compared with less than or equal to 40 microg/L .
	manualset3
209003	6	418095	7	NULL	NULL	0	NULL	 1.1 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	We found a monotonic decrease in mean cycle length with increasing total THM ( TTHM ) level ; at ) 60 microg/L , the adjusted decrement was 1.1 days ( 95 % confidence interval ( CI ) , -1.8 to -0.40 ) , compared with less than or equal to 40 microg/L .
	manualset3
209004	7	418095	7	NULL	NULL	0	NULL	95 % confidence interval ( CI ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We found a monotonic decrease in mean cycle length with increasing total THM ( TTHM ) level ; at ) 60 microg/L , the adjusted decrement was 1.1 days ( 95 % confidence interval ( CI ) , -1.8 to -0.40 ) , compared with less than or equal to 40 microg/L .
	manualset3
209005	8	418095	7	NULL	NULL	0	NULL	-1.8 to -0.40	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	We found a monotonic decrease in mean cycle length with increasing total THM ( TTHM ) level ; at ) 60 microg/L , the adjusted decrement was 1.1 days ( 95 % confidence interval ( CI ) , -1.8 to -0.40 ) , compared with less than or equal to 40 microg/L .
	manualset3
209006	9	418095	7	NULL	NULL	0	NULL	40 microg/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	We found a monotonic decrease in mean cycle length with increasing total THM ( TTHM ) level ; at ) 60 microg/L , the adjusted decrement was 1.1 days ( 95 % confidence interval ( CI ) , -1.8 to -0.40 ) , compared with less than or equal to 40 microg/L .
	manualset3
209007	1	418096	7	NULL	NULL	0	NULL	 mortality rate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The mortality rate was high ( 30 % ) .
	manualset3
209008	2	418096	7	NULL	NULL	0	NULL	high	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The mortality rate was high ( 30 % ) .
	manualset3
209009	3	418096	7	NULL	NULL	0	NULL	 30 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The mortality rate was high ( 30 % ) .
	manualset3
209010	1	418097	7	NULL	NULL	0	NULL	individual scores	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	From the individual scores however , it can be postulated that as a feedback aid to learning , its usefulness may have been limited by the narrow range of ratings given .
	manualset3
209011	2	418097	7	NULL	NULL	0	NULL	feedback	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	From the individual scores however , it can be postulated that as a feedback aid to learning , its usefulness may have been limited by the narrow range of ratings given .
	manualset3
209012	3	418097	7	NULL	NULL	0	NULL	learning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	From the individual scores however , it can be postulated that as a feedback aid to learning , its usefulness may have been limited by the narrow range of ratings given .
	manualset3
209013	4	418097	7	NULL	NULL	0	NULL	 usefulness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	From the individual scores however , it can be postulated that as a feedback aid to learning , its usefulness may have been limited by the narrow range of ratings given .
	manualset3
209014	5	418097	7	NULL	NULL	0	NULL	 narrow range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	From the individual scores however , it can be postulated that as a feedback aid to learning , its usefulness may have been limited by the narrow range of ratings given .
	manualset3
209015	6	418097	7	NULL	NULL	0	NULL	ratings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	From the individual scores however , it can be postulated that as a feedback aid to learning , its usefulness may have been limited by the narrow range of ratings given .
	manualset3
209016	1	418098	7	NULL	NULL	0	NULL	Perivascular infiltrates	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Perivascular infiltrates of MNC as well as neutrophils and eosinophils were the most significant dermal changes , with peak levels at 24-48 hours .
	manualset3
209017	2	418098	7	NULL	NULL	0	NULL	MNC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Perivascular infiltrates of MNC as well as neutrophils and eosinophils were the most significant dermal changes , with peak levels at 24-48 hours .
	manualset3
209018	3	418098	7	NULL	NULL	0	NULL	neutrophils	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Perivascular infiltrates of MNC as well as neutrophils and eosinophils were the most significant dermal changes , with peak levels at 24-48 hours .
	manualset3
209019	4	418098	7	NULL	NULL	0	NULL	 eosinophils	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Perivascular infiltrates of MNC as well as neutrophils and eosinophils were the most significant dermal changes , with peak levels at 24-48 hours .
	manualset3
209020	5	418098	7	NULL	NULL	0	NULL	dermal changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Perivascular infiltrates of MNC as well as neutrophils and eosinophils were the most significant dermal changes , with peak levels at 24-48 hours .
	manualset3
209021	6	418098	7	NULL	NULL	0	NULL	 peak levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Perivascular infiltrates of MNC as well as neutrophils and eosinophils were the most significant dermal changes , with peak levels at 24-48 hours .
	manualset3
209022	7	418098	7	NULL	NULL	0	NULL	24-48 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Perivascular infiltrates of MNC as well as neutrophils and eosinophils were the most significant dermal changes , with peak levels at 24-48 hours .
	manualset3
209023	1	418099	7	NULL	NULL	0	NULL	transfer	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The transfer caused a decrease in the mRNA level of Lhl3 , a homolog of Arabidopsis thaliana Lil3 , within 2 h , followed by gradual restoration depending on the intensity of HL .
	manualset3
209024	2	418099	7	NULL	NULL	0	NULL	decrease	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The transfer caused a decrease in the mRNA level of Lhl3 , a homolog of Arabidopsis thaliana Lil3 , within 2 h , followed by gradual restoration depending on the intensity of HL .
	manualset3
209025	3	418099	7	NULL	NULL	0	NULL	mRNA level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The transfer caused a decrease in the mRNA level of Lhl3 , a homolog of Arabidopsis thaliana Lil3 , within 2 h , followed by gradual restoration depending on the intensity of HL .
	manualset3
209026	4	418099	7	NULL	NULL	0	NULL	Lhl3	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The transfer caused a decrease in the mRNA level of Lhl3 , a homolog of Arabidopsis thaliana Lil3 , within 2 h , followed by gradual restoration depending on the intensity of HL .
	manualset3
209027	5	418099	7	NULL	NULL	0	NULL	homolog	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The transfer caused a decrease in the mRNA level of Lhl3 , a homolog of Arabidopsis thaliana Lil3 , within 2 h , followed by gradual restoration depending on the intensity of HL .
	manualset3
209028	6	418099	7	NULL	NULL	0	NULL	Arabidopsis thaliana	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The transfer caused a decrease in the mRNA level of Lhl3 , a homolog of Arabidopsis thaliana Lil3 , within 2 h , followed by gradual restoration depending on the intensity of HL .
	manualset3
209029	7	418099	7	NULL	NULL	0	NULL	Lil3	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The transfer caused a decrease in the mRNA level of Lhl3 , a homolog of Arabidopsis thaliana Lil3 , within 2 h , followed by gradual restoration depending on the intensity of HL .
	manualset3
209030	8	418099	7	NULL	NULL	0	NULL	 2 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The transfer caused a decrease in the mRNA level of Lhl3 , a homolog of Arabidopsis thaliana Lil3 , within 2 h , followed by gradual restoration depending on the intensity of HL .
	manualset3
209031	9	418099	7	NULL	NULL	0	NULL	 gradual restoration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The transfer caused a decrease in the mRNA level of Lhl3 , a homolog of Arabidopsis thaliana Lil3 , within 2 h , followed by gradual restoration depending on the intensity of HL .
	manualset3
209032	10	418099	7	NULL	NULL	0	NULL	 intensity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The transfer caused a decrease in the mRNA level of Lhl3 , a homolog of Arabidopsis thaliana Lil3 , within 2 h , followed by gradual restoration depending on the intensity of HL .
	manualset3
209033	11	418099	7	NULL	NULL	0	NULL	HL	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The transfer caused a decrease in the mRNA level of Lhl3 , a homolog of Arabidopsis thaliana Lil3 , within 2 h , followed by gradual restoration depending on the intensity of HL .
	manualset3
209034	1	418100	7	NULL	NULL	0	NULL	tested fractions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	All the tested fractions significantly decreased intromission latency and intercopulatory interval and increased intromission frequency and copulatory efficacy ( P & lt ; 0.05 ) as compared to controls .
	manualset3
209035	2	418100	7	NULL	NULL	0	NULL	intromission latency	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	All the tested fractions significantly decreased intromission latency and intercopulatory interval and increased intromission frequency and copulatory efficacy ( P & lt ; 0.05 ) as compared to controls .
	manualset3
209036	3	418100	7	NULL	NULL	0	NULL	intercopulatory interval	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	All the tested fractions significantly decreased intromission latency and intercopulatory interval and increased intromission frequency and copulatory efficacy ( P & lt ; 0.05 ) as compared to controls .
	manualset3
209037	4	418100	7	NULL	NULL	0	NULL	intromission frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All the tested fractions significantly decreased intromission latency and intercopulatory interval and increased intromission frequency and copulatory efficacy ( P & lt ; 0.05 ) as compared to controls .
	manualset3
209038	5	418100	7	NULL	NULL	0	NULL	 copulatory efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All the tested fractions significantly decreased intromission latency and intercopulatory interval and increased intromission frequency and copulatory efficacy ( P & lt ; 0.05 ) as compared to controls .
	manualset3
209039	6	418100	7	NULL	NULL	0	NULL	P & lt ; 0.05	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All the tested fractions significantly decreased intromission latency and intercopulatory interval and increased intromission frequency and copulatory efficacy ( P & lt ; 0.05 ) as compared to controls .
	manualset3
209040	7	418100	7	NULL	NULL	0	NULL	controls	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	All the tested fractions significantly decreased intromission latency and intercopulatory interval and increased intromission frequency and copulatory efficacy ( P & lt ; 0.05 ) as compared to controls .
	manualset3
209041	1	418101	7	NULL	NULL	0	NULL	Twelve patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve patients selected the SCOT II procedure , 11 selected an LHRH agonist , and 5 selected a BTO .
	manualset3
209042	2	418101	7	NULL	NULL	0	NULL	SCOT II procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve patients selected the SCOT II procedure , 11 selected an LHRH agonist , and 5 selected a BTO .
	manualset3
209043	3	418101	7	NULL	NULL	NULL	NULL	11 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Twelve patients selected the SCOT II procedure , 11 selected an LHRH agonist , and 5 selected a BTO .
	manualset3
209044	4	418101	7	NULL	NULL	0	NULL	LHRH agonist	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve patients selected the SCOT II procedure , 11 selected an LHRH agonist , and 5 selected a BTO .
	manualset3
209045	5	418101	7	NULL	NULL	0	NULL	 5 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve patients selected the SCOT II procedure , 11 selected an LHRH agonist , and 5 selected a BTO .
	manualset3
209046	6	418101	7	NULL	NULL	0	NULL	BTO	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve patients selected the SCOT II procedure , 11 selected an LHRH agonist , and 5 selected a BTO .
	manualset3
209047	1	418102	7	NULL	NULL	0	NULL	volume 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The volume and breadth of testing in physicians ' office laboratories ( POLs ) has increased exponentially since passage of the Diagnosis Related Group legislation by Congress in 1983 , an increase made possible by remarkable developments in technology .
	manualset3
209048	2	418102	7	NULL	NULL	0	NULL	breadth	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The volume and breadth of testing in physicians ' office laboratories ( POLs ) has increased exponentially since passage of the Diagnosis Related Group legislation by Congress in 1983 , an increase made possible by remarkable developments in technology .
	manualset3
209049	3	418102	7	NULL	NULL	0	NULL	testing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The volume and breadth of testing in physicians ' office laboratories ( POLs ) has increased exponentially since passage of the Diagnosis Related Group legislation by Congress in 1983 , an increase made possible by remarkable developments in technology .
	manualset3
209050	4	418102	7	NULL	NULL	0	NULL	physicians ' office laboratories ( POLs )	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The volume and breadth of testing in physicians ' office laboratories ( POLs ) has increased exponentially since passage of the Diagnosis Related Group legislation by Congress in 1983 , an increase made possible by remarkable developments in technology .
	manualset3
209051	5	418102	7	NULL	NULL	0	NULL	passage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The volume and breadth of testing in physicians ' office laboratories ( POLs ) has increased exponentially since passage of the Diagnosis Related Group legislation by Congress in 1983 , an increase made possible by remarkable developments in technology .
	manualset3
209052	6	418102	7	NULL	NULL	0	NULL	Diagnosis Related Group legislation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The volume and breadth of testing in physicians ' office laboratories ( POLs ) has increased exponentially since passage of the Diagnosis Related Group legislation by Congress in 1983 , an increase made possible by remarkable developments in technology .
	manualset3
209053	7	418102	7	NULL	NULL	0	NULL	Congress	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The volume and breadth of testing in physicians ' office laboratories ( POLs ) has increased exponentially since passage of the Diagnosis Related Group legislation by Congress in 1983 , an increase made possible by remarkable developments in technology .
	manualset3
209054	8	418102	7	NULL	NULL	0	NULL	1983	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The volume and breadth of testing in physicians ' office laboratories ( POLs ) has increased exponentially since passage of the Diagnosis Related Group legislation by Congress in 1983 , an increase made possible by remarkable developments in technology .
	manualset3
209055	9	418102	7	NULL	NULL	0	NULL	 developments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The volume and breadth of testing in physicians ' office laboratories ( POLs ) has increased exponentially since passage of the Diagnosis Related Group legislation by Congress in 1983 , an increase made possible by remarkable developments in technology .
	manualset3
209056	10	418102	7	NULL	NULL	0	NULL	 technology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The volume and breadth of testing in physicians ' office laboratories ( POLs ) has increased exponentially since passage of the Diagnosis Related Group legislation by Congress in 1983 , an increase made possible by remarkable developments in technology .
	manualset3
209057	11	418102	7	NULL	NULL	0	NULL	increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The volume and breadth of testing in physicians ' office laboratories ( POLs ) has increased exponentially since passage of the Diagnosis Related Group legislation by Congress in 1983 , an increase made possible by remarkable developments in technology .
	manualset3
209058	1	418103	7	NULL	NULL	0	NULL	Phospholipase C isozymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospholipase C isozymes selectively couple to specific neurotransmitter receptors .
	manualset3
209059	2	418103	7	NULL	NULL	0	NULL	neurotransmitter receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospholipase C isozymes selectively couple to specific neurotransmitter receptors .
	manualset3
209060	1	418104	7	NULL	NULL	0	NULL	Tositumomab/iodine -131 tositumomab ( Bexxar )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Tositumomab/iodine -131 tositumomab ( Bexxar ) and ibritumomab tiuxetan ( Zevalin ) are radioimmunoconjugates targeting the CD20 antigen .
	manualset3
209061	2	418104	7	NULL	NULL	0	NULL	ibritumomab tiuxetan ( Zevalin )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Tositumomab/iodine -131 tositumomab ( Bexxar ) and ibritumomab tiuxetan ( Zevalin ) are radioimmunoconjugates targeting the CD20 antigen .
	manualset3
209062	3	418104	7	NULL	NULL	0	NULL	radioimmunoconjugates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Tositumomab/iodine -131 tositumomab ( Bexxar ) and ibritumomab tiuxetan ( Zevalin ) are radioimmunoconjugates targeting the CD20 antigen .
	manualset3
209063	4	418104	7	NULL	NULL	0	NULL	CD20 antigen	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Tositumomab/iodine -131 tositumomab ( Bexxar ) and ibritumomab tiuxetan ( Zevalin ) are radioimmunoconjugates targeting the CD20 antigen .
	manualset3
209064	1	418105	7	NULL	NULL	0	NULL	Birds	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Birds in these floor densities were allowed feeder space of 2.7 , 3.1 , 3.5 , and 4 cm/bird , respectively , and water space of 1.4 , 1.6 , 1.8 , and 2.0 cm/bird , respectively .
	manualset3
209065	2	418105	7	NULL	NULL	0	NULL	 floor densities	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Birds in these floor densities were allowed feeder space of 2.7 , 3.1 , 3.5 , and 4 cm/bird , respectively , and water space of 1.4 , 1.6 , 1.8 , and 2.0 cm/bird , respectively .
	manualset3
209066	3	418105	7	NULL	NULL	0	NULL	 feeder space	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Birds in these floor densities were allowed feeder space of 2.7 , 3.1 , 3.5 , and 4 cm/bird , respectively , and water space of 1.4 , 1.6 , 1.8 , and 2.0 cm/bird , respectively .
	manualset3
209067	4	418105	7	NULL	NULL	0	NULL	2.7 cm/bird	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Birds in these floor densities were allowed feeder space of 2.7 , 3.1 , 3.5 , and 4 cm/bird , respectively , and water space of 1.4 , 1.6 , 1.8 , and 2.0 cm/bird , respectively .
	manualset3
209068	5	418105	7	NULL	NULL	0	NULL	 3.1 cm/bird	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Birds in these floor densities were allowed feeder space of 2.7 , 3.1 , 3.5 , and 4 cm/bird , respectively , and water space of 1.4 , 1.6 , 1.8 , and 2.0 cm/bird , respectively .
	manualset3
209069	6	418105	7	NULL	NULL	0	NULL	4 cm/bird 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Birds in these floor densities were allowed feeder space of 2.7 , 3.1 , 3.5 , and 4 cm/bird , respectively , and water space of 1.4 , 1.6 , 1.8 , and 2.0 cm/bird , respectively .
	manualset3
209070	7	418105	7	NULL	NULL	0	NULL	water space	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Birds in these floor densities were allowed feeder space of 2.7 , 3.1 , 3.5 , and 4 cm/bird , respectively , and water space of 1.4 , 1.6 , 1.8 , and 2.0 cm/bird , respectively .
	manualset3
209071	8	418105	7	NULL	NULL	0	NULL	1.4 cm/bird	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Birds in these floor densities were allowed feeder space of 2.7 , 3.1 , 3.5 , and 4 cm/bird , respectively , and water space of 1.4 , 1.6 , 1.8 , and 2.0 cm/bird , respectively .
	manualset3
209072	9	418105	7	NULL	NULL	0	NULL	1.6 cm/bird	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Birds in these floor densities were allowed feeder space of 2.7 , 3.1 , 3.5 , and 4 cm/bird , respectively , and water space of 1.4 , 1.6 , 1.8 , and 2.0 cm/bird , respectively .
	manualset3
209073	10	418105	7	NULL	NULL	0	NULL	1.8 cm/bird	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Birds in these floor densities were allowed feeder space of 2.7 , 3.1 , 3.5 , and 4 cm/bird , respectively , and water space of 1.4 , 1.6 , 1.8 , and 2.0 cm/bird , respectively .
	manualset3
209074	11	418105	7	NULL	NULL	0	NULL	2.0 cm/bird	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Birds in these floor densities were allowed feeder space of 2.7 , 3.1 , 3.5 , and 4 cm/bird , respectively , and water space of 1.4 , 1.6 , 1.8 , and 2.0 cm/bird , respectively .
	manualset3
209075	12	418105	7	NULL	NULL	0	NULL	3.5 cm/bird	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Birds in these floor densities were allowed feeder space of 2.7 , 3.1 , 3.5 , and 4 cm/bird , respectively , and water space of 1.4 , 1.6 , 1.8 , and 2.0 cm/bird , respectively .
	manualset3
209076	1	418106	7	NULL	NULL	0	NULL	Penaincisalia sigsiga 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Penaincisalia sigsiga ( Blint et al ) , P. cillutincarae ( Draudt ) , P. atymna ( Hewitson ) and P. loxurina ( C. Felder & R. Felder ) were easily delimited as the morphological , geographic and molecular data were congruent .
	manualset3
209077	2	418106	7	NULL	NULL	0	NULL	Blint et al 	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	Penaincisalia sigsiga ( Blint et al ) , P. cillutincarae ( Draudt ) , P. atymna ( Hewitson ) and P. loxurina ( C. Felder & R. Felder ) were easily delimited as the morphological , geographic and molecular data were congruent .
	manualset3
209078	3	418106	7	NULL	NULL	0	NULL	 P. cillutincarae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Penaincisalia sigsiga ( Blint et al ) , P. cillutincarae ( Draudt ) , P. atymna ( Hewitson ) and P. loxurina ( C. Felder & R. Felder ) were easily delimited as the morphological , geographic and molecular data were congruent .
	manualset3
209079	4	418106	7	NULL	NULL	0	NULL	Draudt	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	Penaincisalia sigsiga ( Blint et al ) , P. cillutincarae ( Draudt ) , P. atymna ( Hewitson ) and P. loxurina ( C. Felder & R. Felder ) were easily delimited as the morphological , geographic and molecular data were congruent .
	manualset3
209080	5	418106	7	NULL	NULL	0	NULL	P. atymna	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Penaincisalia sigsiga ( Blint et al ) , P. cillutincarae ( Draudt ) , P. atymna ( Hewitson ) and P. loxurina ( C. Felder & R. Felder ) were easily delimited as the morphological , geographic and molecular data were congruent .
	manualset3
209081	6	418106	7	NULL	NULL	0	NULL	 Hewitson	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	Penaincisalia sigsiga ( Blint et al ) , P. cillutincarae ( Draudt ) , P. atymna ( Hewitson ) and P. loxurina ( C. Felder & R. Felder ) were easily delimited as the morphological , geographic and molecular data were congruent .
	manualset3
209082	7	418106	7	NULL	NULL	0	NULL	P. loxurina	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Penaincisalia sigsiga ( Blint et al ) , P. cillutincarae ( Draudt ) , P. atymna ( Hewitson ) and P. loxurina ( C. Felder & R. Felder ) were easily delimited as the morphological , geographic and molecular data were congruent .
	manualset3
209083	8	418106	7	NULL	NULL	0	NULL	C. Felder & R. Felder	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	Penaincisalia sigsiga ( Blint et al ) , P. cillutincarae ( Draudt ) , P. atymna ( Hewitson ) and P. loxurina ( C. Felder & R. Felder ) were easily delimited as the morphological , geographic and molecular data were congruent .
	manualset3
209084	9	418106	7	NULL	NULL	0	NULL	morphological data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Penaincisalia sigsiga ( Blint et al ) , P. cillutincarae ( Draudt ) , P. atymna ( Hewitson ) and P. loxurina ( C. Felder & R. Felder ) were easily delimited as the morphological , geographic and molecular data were congruent .
	manualset3
209085	10	418106	7	NULL	NULL	0	NULL	geographic data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Penaincisalia sigsiga ( Blint et al ) , P. cillutincarae ( Draudt ) , P. atymna ( Hewitson ) and P. loxurina ( C. Felder & R. Felder ) were easily delimited as the morphological , geographic and molecular data were congruent .
	manualset3
209086	11	418106	7	NULL	NULL	0	NULL	molecular data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Penaincisalia sigsiga ( Blint et al ) , P. cillutincarae ( Draudt ) , P. atymna ( Hewitson ) and P. loxurina ( C. Felder & R. Felder ) were easily delimited as the morphological , geographic and molecular data were congruent .
	manualset3
209087	1	418107	7	NULL	NULL	0	NULL	Culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	( Culture of Pityrosporum ovale on oleic acid medium ) .
	manualset3
209088	2	418107	7	NULL	NULL	0	NULL	Pityrosporum ovale	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Culture of Pityrosporum ovale on oleic acid medium ) .
	manualset3
209089	3	418107	7	NULL	NULL	0	NULL	oleic acid medium	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	( Culture of Pityrosporum ovale on oleic acid medium ) .
	manualset3
209090	1	418108	7	NULL	NULL	0	NULL	Nurses	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurses provide early detection and coordinate with other members of the healthcare team to initiate a plan of care that includes prompt treatment of delirium to reduce the signs and symptoms , duration , and potential adverse sequelae of this disorder .
	manualset3
209091	2	418108	7	NULL	NULL	0	NULL	 early detection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurses provide early detection and coordinate with other members of the healthcare team to initiate a plan of care that includes prompt treatment of delirium to reduce the signs and symptoms , duration , and potential adverse sequelae of this disorder .
	manualset3
209092	3	418108	7	NULL	NULL	0	NULL	members	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurses provide early detection and coordinate with other members of the healthcare team to initiate a plan of care that includes prompt treatment of delirium to reduce the signs and symptoms , duration , and potential adverse sequelae of this disorder .
	manualset3
209093	4	418108	7	NULL	NULL	0	NULL	healthcare team	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurses provide early detection and coordinate with other members of the healthcare team to initiate a plan of care that includes prompt treatment of delirium to reduce the signs and symptoms , duration , and potential adverse sequelae of this disorder .
	manualset3
209094	5	418108	7	NULL	NULL	0	NULL	plan of care	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurses provide early detection and coordinate with other members of the healthcare team to initiate a plan of care that includes prompt treatment of delirium to reduce the signs and symptoms , duration , and potential adverse sequelae of this disorder .
	manualset3
209095	6	418108	7	NULL	NULL	0	NULL	 treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurses provide early detection and coordinate with other members of the healthcare team to initiate a plan of care that includes prompt treatment of delirium to reduce the signs and symptoms , duration , and potential adverse sequelae of this disorder .
	manualset3
209096	7	418108	7	NULL	NULL	0	NULL	 delirium	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurses provide early detection and coordinate with other members of the healthcare team to initiate a plan of care that includes prompt treatment of delirium to reduce the signs and symptoms , duration , and potential adverse sequelae of this disorder .
	manualset3
209097	8	418108	7	NULL	NULL	0	NULL	 signs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurses provide early detection and coordinate with other members of the healthcare team to initiate a plan of care that includes prompt treatment of delirium to reduce the signs and symptoms , duration , and potential adverse sequelae of this disorder .
	manualset3
209098	9	418108	7	NULL	NULL	0	NULL	symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurses provide early detection and coordinate with other members of the healthcare team to initiate a plan of care that includes prompt treatment of delirium to reduce the signs and symptoms , duration , and potential adverse sequelae of this disorder .
	manualset3
209099	10	418108	7	NULL	NULL	0	NULL	 duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurses provide early detection and coordinate with other members of the healthcare team to initiate a plan of care that includes prompt treatment of delirium to reduce the signs and symptoms , duration , and potential adverse sequelae of this disorder .
	manualset3
209100	11	418108	7	NULL	NULL	0	NULL	potential adverse sequelae	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurses provide early detection and coordinate with other members of the healthcare team to initiate a plan of care that includes prompt treatment of delirium to reduce the signs and symptoms , duration , and potential adverse sequelae of this disorder .
	manualset3
209101	12	418108	7	NULL	NULL	0	NULL	 disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurses provide early detection and coordinate with other members of the healthcare team to initiate a plan of care that includes prompt treatment of delirium to reduce the signs and symptoms , duration , and potential adverse sequelae of this disorder .
	manualset3
209102	1	418109	7	NULL	NULL	0	NULL	indirect fluorescent staining	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	By using indirect fluorescent staining with anti-actin rabbit serum , direct evidence was obtained that interaction with the cytoskeleton of HEp-2 cells is necessary for invasion .
	manualset3
209103	2	418109	7	NULL	NULL	0	NULL	anti-actin rabbit serum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	By using indirect fluorescent staining with anti-actin rabbit serum , direct evidence was obtained that interaction with the cytoskeleton of HEp-2 cells is necessary for invasion .
	manualset3
209104	3	418109	7	NULL	NULL	0	NULL	direct evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	By using indirect fluorescent staining with anti-actin rabbit serum , direct evidence was obtained that interaction with the cytoskeleton of HEp-2 cells is necessary for invasion .
	manualset3
209105	4	418109	7	NULL	NULL	0	NULL	interaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	By using indirect fluorescent staining with anti-actin rabbit serum , direct evidence was obtained that interaction with the cytoskeleton of HEp-2 cells is necessary for invasion .
	manualset3
209106	5	418109	7	NULL	NULL	0	NULL	 cytoskeleton	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	By using indirect fluorescent staining with anti-actin rabbit serum , direct evidence was obtained that interaction with the cytoskeleton of HEp-2 cells is necessary for invasion .
	manualset3
209107	6	418109	7	NULL	NULL	0	NULL	HEp-2 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	By using indirect fluorescent staining with anti-actin rabbit serum , direct evidence was obtained that interaction with the cytoskeleton of HEp-2 cells is necessary for invasion .
	manualset3
209108	7	418109	7	NULL	NULL	0	NULL	invasion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	By using indirect fluorescent staining with anti-actin rabbit serum , direct evidence was obtained that interaction with the cytoskeleton of HEp-2 cells is necessary for invasion .
	manualset3
209109	1	418110	7	NULL	NULL	0	NULL	2-Chloro-N - ( 4-nitro-benzo-yl ) benzene-sulfonamide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	2-Chloro-N - ( 4-nitro-benzo-yl ) benzene-sulfonamide .
	manualset3
209110	1	418111	7	NULL	NULL	0	NULL	Conclusions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions Influenza B accounts for about 8percnt ; of the incidence of invasive S. pyogenes infections , over and above any effect associated with modellable seasonal and long-term trends .
	manualset3
209111	2	418111	7	NULL	NULL	0	NULL	Influenza B	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions Influenza B accounts for about 8percnt ; of the incidence of invasive S. pyogenes infections , over and above any effect associated with modellable seasonal and long-term trends .
	manualset3
209112	3	418111	7	NULL	NULL	0	NULL	8percnt	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions Influenza B accounts for about 8percnt ; of the incidence of invasive S. pyogenes infections , over and above any effect associated with modellable seasonal and long-term trends .
	manualset3
209113	4	418111	7	NULL	NULL	0	NULL	incidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions Influenza B accounts for about 8percnt ; of the incidence of invasive S. pyogenes infections , over and above any effect associated with modellable seasonal and long-term trends .
	manualset3
209114	5	418111	7	NULL	NULL	0	NULL	invasive S. pyogenes infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions Influenza B accounts for about 8percnt ; of the incidence of invasive S. pyogenes infections , over and above any effect associated with modellable seasonal and long-term trends .
	manualset3
209115	6	418111	7	NULL	NULL	0	NULL	modellable seasonal trends	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions Influenza B accounts for about 8percnt ; of the incidence of invasive S. pyogenes infections , over and above any effect associated with modellable seasonal and long-term trends .
	manualset3
209116	7	418111	7	NULL	NULL	0	NULL	long-term trends	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions Influenza B accounts for about 8percnt ; of the incidence of invasive S. pyogenes infections , over and above any effect associated with modellable seasonal and long-term trends .
	manualset3
209117	1	418112	7	NULL	NULL	0	NULL	hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In hepatocytes , as in other cell types , Ca ( 2 + ) signaling is subject to complex regulations , which result largely from the intrinsic characteristics of the different inositol 1 , 4 , 5-trisphosphate receptor ( InsP ( 3 ) R ) isoforms and from their interactions with other proteins .
	manualset3
209118	2	418112	7	NULL	NULL	0	NULL	cell types	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In hepatocytes , as in other cell types , Ca ( 2 + ) signaling is subject to complex regulations , which result largely from the intrinsic characteristics of the different inositol 1 , 4 , 5-trisphosphate receptor ( InsP ( 3 ) R ) isoforms and from their interactions with other proteins .
	manualset3
209119	3	418112	7	NULL	NULL	0	NULL	Ca ( 2 + ) signaling 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In hepatocytes , as in other cell types , Ca ( 2 + ) signaling is subject to complex regulations , which result largely from the intrinsic characteristics of the different inositol 1 , 4 , 5-trisphosphate receptor ( InsP ( 3 ) R ) isoforms and from their interactions with other proteins .
	manualset3
209120	4	418112	7	NULL	NULL	0	NULL	complex regulations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In hepatocytes , as in other cell types , Ca ( 2 + ) signaling is subject to complex regulations , which result largely from the intrinsic characteristics of the different inositol 1 , 4 , 5-trisphosphate receptor ( InsP ( 3 ) R ) isoforms and from their interactions with other proteins .
	manualset3
209121	5	418112	7	NULL	NULL	0	NULL	 intrinsic characteristics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In hepatocytes , as in other cell types , Ca ( 2 + ) signaling is subject to complex regulations , which result largely from the intrinsic characteristics of the different inositol 1 , 4 , 5-trisphosphate receptor ( InsP ( 3 ) R ) isoforms and from their interactions with other proteins .
	manualset3
209122	6	418112	7	NULL	NULL	0	NULL	 inositol 1 , 4 , 5-trisphosphate receptor ( InsP ( 3 ) R ) isoforms	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In hepatocytes , as in other cell types , Ca ( 2 + ) signaling is subject to complex regulations , which result largely from the intrinsic characteristics of the different inositol 1 , 4 , 5-trisphosphate receptor ( InsP ( 3 ) R ) isoforms and from their interactions with other proteins .
	manualset3
209123	7	418112	7	NULL	NULL	0	NULL	interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In hepatocytes , as in other cell types , Ca ( 2 + ) signaling is subject to complex regulations , which result largely from the intrinsic characteristics of the different inositol 1 , 4 , 5-trisphosphate receptor ( InsP ( 3 ) R ) isoforms and from their interactions with other proteins .
	manualset3
209124	8	418112	7	NULL	NULL	0	NULL	 proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In hepatocytes , as in other cell types , Ca ( 2 + ) signaling is subject to complex regulations , which result largely from the intrinsic characteristics of the different inositol 1 , 4 , 5-trisphosphate receptor ( InsP ( 3 ) R ) isoforms and from their interactions with other proteins .
	manualset3
209125	1	418113	7	NULL	NULL	0	NULL	Lipemia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Lipemia and lipemic fractions in various periods of pregnancy ) .
	manualset3
209126	2	418113	7	NULL	NULL	0	NULL	lipemic fractions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Lipemia and lipemic fractions in various periods of pregnancy ) .
	manualset3
209127	3	418113	7	NULL	NULL	0	NULL	 periods	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	( Lipemia and lipemic fractions in various periods of pregnancy ) .
	manualset3
209128	4	418113	7	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Lipemia and lipemic fractions in various periods of pregnancy ) .
	manualset3
209129	1	418114	7	NULL	NULL	0	NULL	Distamycin A	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Distamycin A and its analogs as agents for blocking of endo R. EcoRI activity .
	manualset3
209130	2	418114	7	NULL	NULL	0	NULL	analogs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Distamycin A and its analogs as agents for blocking of endo R. EcoRI activity .
	manualset3
209131	3	418114	7	NULL	NULL	0	NULL	agents	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Distamycin A and its analogs as agents for blocking of endo R. EcoRI activity .
	manualset3
209132	4	418114	7	NULL	NULL	0	NULL	 blocking 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Distamycin A and its analogs as agents for blocking of endo R. EcoRI activity .
	manualset3
209133	5	418114	7	NULL	NULL	0	NULL	endo R. EcoRI activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Distamycin A and its analogs as agents for blocking of endo R. EcoRI activity .
	manualset3
209134	1	418115	7	NULL	NULL	0	NULL	All steps	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	All steps of the procedure , such as solid sample dissolution , pre-reduction to the suitable oxidation state , vapor generation , transport and atomization have been designed and optimised taking into account the concomitant presence of all the analytes considered .
	manualset3
209135	2	418115	7	NULL	NULL	0	NULL	 procedure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	All steps of the procedure , such as solid sample dissolution , pre-reduction to the suitable oxidation state , vapor generation , transport and atomization have been designed and optimised taking into account the concomitant presence of all the analytes considered .
	manualset3
209136	3	418115	7	NULL	NULL	NULL	NULL	solid sample dissolution	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	All steps of the procedure , such as solid sample dissolution , pre-reduction to the suitable oxidation state , vapor generation , transport and atomization have been designed and optimised taking into account the concomitant presence of all the analytes considered .
	manualset3
209137	4	418115	7	NULL	NULL	0	NULL	pre-reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	All steps of the procedure , such as solid sample dissolution , pre-reduction to the suitable oxidation state , vapor generation , transport and atomization have been designed and optimised taking into account the concomitant presence of all the analytes considered .
	manualset3
209138	5	418115	7	NULL	NULL	0	NULL	suitable oxidation state	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All steps of the procedure , such as solid sample dissolution , pre-reduction to the suitable oxidation state , vapor generation , transport and atomization have been designed and optimised taking into account the concomitant presence of all the analytes considered .
	manualset3
209139	6	418115	7	NULL	NULL	0	NULL	vapor generation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	All steps of the procedure , such as solid sample dissolution , pre-reduction to the suitable oxidation state , vapor generation , transport and atomization have been designed and optimised taking into account the concomitant presence of all the analytes considered .
	manualset3
209140	7	418115	7	NULL	NULL	0	NULL	transport	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	All steps of the procedure , such as solid sample dissolution , pre-reduction to the suitable oxidation state , vapor generation , transport and atomization have been designed and optimised taking into account the concomitant presence of all the analytes considered .
	manualset3
209141	8	418115	7	NULL	NULL	0	NULL	atomization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	All steps of the procedure , such as solid sample dissolution , pre-reduction to the suitable oxidation state , vapor generation , transport and atomization have been designed and optimised taking into account the concomitant presence of all the analytes considered .
	manualset3
209142	9	418115	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	All steps of the procedure , such as solid sample dissolution , pre-reduction to the suitable oxidation state , vapor generation , transport and atomization have been designed and optimised taking into account the concomitant presence of all the analytes considered .
	manualset3
209143	10	418115	7	NULL	NULL	0	NULL	analytes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All steps of the procedure , such as solid sample dissolution , pre-reduction to the suitable oxidation state , vapor generation , transport and atomization have been designed and optimised taking into account the concomitant presence of all the analytes considered .
	manualset3
209144	1	418116	7	NULL	NULL	0	NULL	Free N protein content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Free N protein content was compared in the two types of rabies vaccine currently used in humans : suckling mouse brain ( SMB ) vaccine prepared from rabies virus-infected brain tissue , and tissue culture ( TC ) vaccine prepared from supernatants of rabies virus-infected cells .
	manualset3
209145	2	418116	7	NULL	NULL	0	NULL	 two types	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Free N protein content was compared in the two types of rabies vaccine currently used in humans : suckling mouse brain ( SMB ) vaccine prepared from rabies virus-infected brain tissue , and tissue culture ( TC ) vaccine prepared from supernatants of rabies virus-infected cells .
	manualset3
209146	3	418116	7	NULL	NULL	0	NULL	 rabies vaccine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Free N protein content was compared in the two types of rabies vaccine currently used in humans : suckling mouse brain ( SMB ) vaccine prepared from rabies virus-infected brain tissue , and tissue culture ( TC ) vaccine prepared from supernatants of rabies virus-infected cells .
	manualset3
209147	4	418116	7	NULL	NULL	0	NULL	humans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Free N protein content was compared in the two types of rabies vaccine currently used in humans : suckling mouse brain ( SMB ) vaccine prepared from rabies virus-infected brain tissue , and tissue culture ( TC ) vaccine prepared from supernatants of rabies virus-infected cells .
	manualset3
209148	5	418116	7	NULL	NULL	0	NULL	suckling mouse brain ( SMB ) vaccine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Free N protein content was compared in the two types of rabies vaccine currently used in humans : suckling mouse brain ( SMB ) vaccine prepared from rabies virus-infected brain tissue , and tissue culture ( TC ) vaccine prepared from supernatants of rabies virus-infected cells .
	manualset3
209149	6	418116	7	NULL	NULL	0	NULL	rabies virus-infected brain tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Free N protein content was compared in the two types of rabies vaccine currently used in humans : suckling mouse brain ( SMB ) vaccine prepared from rabies virus-infected brain tissue , and tissue culture ( TC ) vaccine prepared from supernatants of rabies virus-infected cells .
	manualset3
209150	7	418116	7	NULL	NULL	0	NULL	tissue culture ( TC ) vaccine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Free N protein content was compared in the two types of rabies vaccine currently used in humans : suckling mouse brain ( SMB ) vaccine prepared from rabies virus-infected brain tissue , and tissue culture ( TC ) vaccine prepared from supernatants of rabies virus-infected cells .
	manualset3
209151	8	418116	7	NULL	NULL	0	NULL	supernatants 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Free N protein content was compared in the two types of rabies vaccine currently used in humans : suckling mouse brain ( SMB ) vaccine prepared from rabies virus-infected brain tissue , and tissue culture ( TC ) vaccine prepared from supernatants of rabies virus-infected cells .
	manualset3
209152	9	418116	7	NULL	NULL	0	NULL	rabies virus-infected cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Free N protein content was compared in the two types of rabies vaccine currently used in humans : suckling mouse brain ( SMB ) vaccine prepared from rabies virus-infected brain tissue , and tissue culture ( TC ) vaccine prepared from supernatants of rabies virus-infected cells .
	manualset3
209153	1	418117	7	NULL	NULL	0	NULL	Effect 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Effect of phenobarbital and carbon tetrachloride on dehydrocholate induced choleresis in the guinea-pig .
	manualset3
209154	2	418117	7	NULL	NULL	0	NULL	 phenobarbital	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Effect of phenobarbital and carbon tetrachloride on dehydrocholate induced choleresis in the guinea-pig .
	manualset3
209155	3	418117	7	NULL	NULL	NULL	NULL	carbon tetrachloride 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of phenobarbital and carbon tetrachloride on dehydrocholate induced choleresis in the guinea-pig .
	manualset3
209156	5	418117	7	NULL	NULL	NULL	NULL	guinea-pig	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of phenobarbital and carbon tetrachloride on dehydrocholate induced choleresis in the guinea-pig .
	manualset3
209819	4	418117	7	NULL	NULL	0	NULL	dehydrocholate induced choleresis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Effect of phenobarbital and carbon tetrachloride on dehydrocholate induced choleresis in the guinea-pig .
	manualset3
209157	1	418118	7	NULL	NULL	0	NULL	Comparable results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparable results were obtained in male rats , except that testosterone did not significantly attenuate ER mRNA hybridization in the VMHvl until after 3 days of hormone treatment , and only a minor decrease was noted in the ARH , which was not statistically significant .
	manualset3
209158	2	418118	7	NULL	NULL	0	NULL	male rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparable results were obtained in male rats , except that testosterone did not significantly attenuate ER mRNA hybridization in the VMHvl until after 3 days of hormone treatment , and only a minor decrease was noted in the ARH , which was not statistically significant .
	manualset3
209159	3	418118	7	NULL	NULL	0	NULL	testosterone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparable results were obtained in male rats , except that testosterone did not significantly attenuate ER mRNA hybridization in the VMHvl until after 3 days of hormone treatment , and only a minor decrease was noted in the ARH , which was not statistically significant .
	manualset3
209160	4	418118	7	NULL	NULL	0	NULL	ER mRNA hybridization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparable results were obtained in male rats , except that testosterone did not significantly attenuate ER mRNA hybridization in the VMHvl until after 3 days of hormone treatment , and only a minor decrease was noted in the ARH , which was not statistically significant .
	manualset3
209161	5	418118	7	NULL	NULL	0	NULL	VMHvl 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparable results were obtained in male rats , except that testosterone did not significantly attenuate ER mRNA hybridization in the VMHvl until after 3 days of hormone treatment , and only a minor decrease was noted in the ARH , which was not statistically significant .
	manualset3
209162	6	418118	7	NULL	NULL	0	NULL	 3 days 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparable results were obtained in male rats , except that testosterone did not significantly attenuate ER mRNA hybridization in the VMHvl until after 3 days of hormone treatment , and only a minor decrease was noted in the ARH , which was not statistically significant .
	manualset3
209163	7	418118	7	NULL	NULL	0	NULL	hormone treatment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparable results were obtained in male rats , except that testosterone did not significantly attenuate ER mRNA hybridization in the VMHvl until after 3 days of hormone treatment , and only a minor decrease was noted in the ARH , which was not statistically significant .
	manualset3
209164	8	418118	7	NULL	NULL	0	NULL	 minor decrease 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparable results were obtained in male rats , except that testosterone did not significantly attenuate ER mRNA hybridization in the VMHvl until after 3 days of hormone treatment , and only a minor decrease was noted in the ARH , which was not statistically significant .
	manualset3
209165	9	418118	7	NULL	NULL	0	NULL	ARH	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparable results were obtained in male rats , except that testosterone did not significantly attenuate ER mRNA hybridization in the VMHvl until after 3 days of hormone treatment , and only a minor decrease was noted in the ARH , which was not statistically significant .
	manualset3
209166	1	418119	7	NULL	NULL	NULL	NULL	expanding research field 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The expanding research field of cancer stem-cell biology may offer a novel clinical apparatus to the diagnosis and treatment of cancer .
	manualset3
209167	2	418119	7	NULL	NULL	0	NULL	cancer stem-cell biology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The expanding research field of cancer stem-cell biology may offer a novel clinical apparatus to the diagnosis and treatment of cancer .
	manualset3
209168	3	418119	7	NULL	NULL	0	NULL	novel clinical apparatus	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The expanding research field of cancer stem-cell biology may offer a novel clinical apparatus to the diagnosis and treatment of cancer .
	manualset3
209169	4	418119	7	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The expanding research field of cancer stem-cell biology may offer a novel clinical apparatus to the diagnosis and treatment of cancer .
	manualset3
209170	5	418119	7	NULL	NULL	0	NULL	 treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The expanding research field of cancer stem-cell biology may offer a novel clinical apparatus to the diagnosis and treatment of cancer .
	manualset3
209171	6	418119	7	NULL	NULL	0	NULL	 cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The expanding research field of cancer stem-cell biology may offer a novel clinical apparatus to the diagnosis and treatment of cancer .
	manualset3
209172	1	418120	7	NULL	NULL	NULL	NULL	model	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We find that a model in which the infected cell death rate is dependent on the infected cell density does not suffer this shortcoming .
	manualset3
209173	2	418120	7	NULL	NULL	NULL	NULL	 infected cell death rate	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We find that a model in which the infected cell death rate is dependent on the infected cell density does not suffer this shortcoming .
	manualset3
209174	3	418120	7	NULL	NULL	NULL	NULL	infected cell density	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We find that a model in which the infected cell death rate is dependent on the infected cell density does not suffer this shortcoming .
	manualset3
209820	4	418120	7	NULL	NULL	0	NULL	shortcoming	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We find that a model in which the infected cell death rate is dependent on the infected cell density does not suffer this shortcoming .
	manualset3
209175	1	418121	7	NULL	NULL	0	NULL	DOC-2 / DAB2	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	DOC-2 / DAB2 is a member of the disable gene family with tumor-inhibitory activity .
	manualset3
209176	2	418121	7	NULL	NULL	0	NULL	member	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	DOC-2 / DAB2 is a member of the disable gene family with tumor-inhibitory activity .
	manualset3
209177	3	418121	7	NULL	NULL	0	NULL	disable gene family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	DOC-2 / DAB2 is a member of the disable gene family with tumor-inhibitory activity .
	manualset3
209178	4	418121	7	NULL	NULL	0	NULL	 tumor-inhibitory activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	DOC-2 / DAB2 is a member of the disable gene family with tumor-inhibitory activity .
	manualset3
209179	1	418122	7	NULL	NULL	0	NULL	Activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity of MAO in some areas of 25-month old , diestrus rats was altered as compared to young , cycling rats ; however , ageing was not associated with widespread changes in MAO activity .
	manualset3
209180	2	418122	7	NULL	NULL	0	NULL	MAO	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity of MAO in some areas of 25-month old , diestrus rats was altered as compared to young , cycling rats ; however , ageing was not associated with widespread changes in MAO activity .
	manualset3
209181	3	418122	7	NULL	NULL	0	NULL	25-month old	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity of MAO in some areas of 25-month old , diestrus rats was altered as compared to young , cycling rats ; however , ageing was not associated with widespread changes in MAO activity .
	manualset3
209182	4	418122	7	NULL	NULL	0	NULL	diestrus rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity of MAO in some areas of 25-month old , diestrus rats was altered as compared to young , cycling rats ; however , ageing was not associated with widespread changes in MAO activity .
	manualset3
209183	5	418122	7	NULL	NULL	0	NULL	young , cycling rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity of MAO in some areas of 25-month old , diestrus rats was altered as compared to young , cycling rats ; however , ageing was not associated with widespread changes in MAO activity .
	manualset3
209184	6	418122	7	NULL	NULL	0	NULL	ageing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity of MAO in some areas of 25-month old , diestrus rats was altered as compared to young , cycling rats ; however , ageing was not associated with widespread changes in MAO activity .
	manualset3
209185	7	418122	7	NULL	NULL	0	NULL	changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity of MAO in some areas of 25-month old , diestrus rats was altered as compared to young , cycling rats ; however , ageing was not associated with widespread changes in MAO activity .
	manualset3
209186	8	418122	7	NULL	NULL	0	NULL	MAO activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity of MAO in some areas of 25-month old , diestrus rats was altered as compared to young , cycling rats ; however , ageing was not associated with widespread changes in MAO activity .
	manualset3
209187	1	418123	7	NULL	NULL	0	NULL	peak outward ( K ) current	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Both the peak outward ( K ) current and the maximum outward ( K ) conductance were reduced by 25 and 29 % , resp .
	manualset3
209188	2	418123	7	NULL	NULL	0	NULL	maximum outward ( K ) conductance	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Both the peak outward ( K ) current and the maximum outward ( K ) conductance were reduced by 25 and 29 % , resp .
	manualset3
209189	3	418123	7	NULL	NULL	0	NULL	25%	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Both the peak outward ( K ) current and the maximum outward ( K ) conductance were reduced by 25 and 29 % , resp .
	manualset3
209190	4	418123	7	NULL	NULL	0	NULL	29 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Both the peak outward ( K ) current and the maximum outward ( K ) conductance were reduced by 25 and 29 % , resp .
	manualset3
209191	1	418124	7	NULL	NULL	0	NULL	procreation rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The procreation rate in couples with affected children is lower in high risk cases and depends also on the family composition .
	manualset3
209192	2	418124	7	NULL	NULL	0	NULL	couples	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The procreation rate in couples with affected children is lower in high risk cases and depends also on the family composition .
	manualset3
209193	3	418124	7	NULL	NULL	0	NULL	affected children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The procreation rate in couples with affected children is lower in high risk cases and depends also on the family composition .
	manualset3
209194	4	418124	7	NULL	NULL	0	NULL	high risk cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The procreation rate in couples with affected children is lower in high risk cases and depends also on the family composition .
	manualset3
209195	5	418124	7	NULL	NULL	0	NULL	family composition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The procreation rate in couples with affected children is lower in high risk cases and depends also on the family composition .
	manualset3
209196	1	418125	7	NULL	NULL	0	NULL	Solution structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Solution structure and interaction of cupiennin 1a , a spider venom peptide , with phospholipid bilayers .
	manualset3
209197	2	418125	7	NULL	NULL	0	NULL	interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Solution structure and interaction of cupiennin 1a , a spider venom peptide , with phospholipid bilayers .
	manualset3
209198	3	418125	7	NULL	NULL	0	NULL	cupiennin 1a 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Solution structure and interaction of cupiennin 1a , a spider venom peptide , with phospholipid bilayers .
	manualset3
209199	4	418125	7	NULL	NULL	0	NULL	spider venom peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Solution structure and interaction of cupiennin 1a , a spider venom peptide , with phospholipid bilayers .
	manualset3
209200	5	418125	7	NULL	NULL	0	NULL	phospholipid bilayers	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Solution structure and interaction of cupiennin 1a , a spider venom peptide , with phospholipid bilayers .
	manualset3
209201	1	418126	7	NULL	NULL	0	NULL	 protein product 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein product of the cro gene consists of 61 amino acid residues , and that of c1 , 92 amino acid residues .
	manualset3
209202	2	418126	7	NULL	NULL	0	NULL	 cro gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein product of the cro gene consists of 61 amino acid residues , and that of c1 , 92 amino acid residues .
	manualset3
209203	3	418126	7	NULL	NULL	0	NULL	 61 amino acid residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein product of the cro gene consists of 61 amino acid residues , and that of c1 , 92 amino acid residues .
	manualset3
209204	4	418126	7	NULL	NULL	0	NULL	c1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein product of the cro gene consists of 61 amino acid residues , and that of c1 , 92 amino acid residues .
	manualset3
209205	5	418126	7	NULL	NULL	0	NULL	92 amino acid residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein product of the cro gene consists of 61 amino acid residues , and that of c1 , 92 amino acid residues .
	manualset3
209206	1	418127	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the results are reproducible within 5 per cent , which means that the method could be of value in the management of metabolic bone diseases .
	manualset3
209207	2	418127	7	NULL	NULL	0	NULL	 5 per cent 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the results are reproducible within 5 per cent , which means that the method could be of value in the management of metabolic bone diseases .
	manualset3
209208	3	418127	7	NULL	NULL	0	NULL	method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the results are reproducible within 5 per cent , which means that the method could be of value in the management of metabolic bone diseases .
	manualset3
209209	4	418127	7	NULL	NULL	0	NULL	value	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the results are reproducible within 5 per cent , which means that the method could be of value in the management of metabolic bone diseases .
	manualset3
209210	5	418127	7	NULL	NULL	0	NULL	management 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the results are reproducible within 5 per cent , which means that the method could be of value in the management of metabolic bone diseases .
	manualset3
209211	6	418127	7	NULL	NULL	0	NULL	metabolic bone diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the results are reproducible within 5 per cent , which means that the method could be of value in the management of metabolic bone diseases .
	manualset3
209212	1	418128	7	NULL	NULL	0	NULL	stereotaxic methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	With stereotaxic methods under chloralose anesthesia the hypothalami of naturally estrous or estrogen-gonadotropin-primed queens were stimulated bilaterally in one of the following regions : medial basal hypothalamus including the premamillary area ( MBH ) and the anterior hypothalamus including both medial and lateral divisions ( AH , MAH , LAH ) .
	manualset3
209213	2	418128	7	NULL	NULL	0	NULL	chloralose anesthesia	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	With stereotaxic methods under chloralose anesthesia the hypothalami of naturally estrous or estrogen-gonadotropin-primed queens were stimulated bilaterally in one of the following regions : medial basal hypothalamus including the premamillary area ( MBH ) and the anterior hypothalamus including both medial and lateral divisions ( AH , MAH , LAH ) .
	manualset3
209214	3	418128	7	NULL	NULL	0	NULL	hypothalami 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	With stereotaxic methods under chloralose anesthesia the hypothalami of naturally estrous or estrogen-gonadotropin-primed queens were stimulated bilaterally in one of the following regions : medial basal hypothalamus including the premamillary area ( MBH ) and the anterior hypothalamus including both medial and lateral divisions ( AH , MAH , LAH ) .
	manualset3
209215	4	418128	7	NULL	NULL	0	NULL	naturally estrous-primed queens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	With stereotaxic methods under chloralose anesthesia the hypothalami of naturally estrous or estrogen-gonadotropin-primed queens were stimulated bilaterally in one of the following regions : medial basal hypothalamus including the premamillary area ( MBH ) and the anterior hypothalamus including both medial and lateral divisions ( AH , MAH , LAH ) .
	manualset3
209216	5	418128	7	NULL	NULL	0	NULL	estrogen-gonadotropin-primed queens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	With stereotaxic methods under chloralose anesthesia the hypothalami of naturally estrous or estrogen-gonadotropin-primed queens were stimulated bilaterally in one of the following regions : medial basal hypothalamus including the premamillary area ( MBH ) and the anterior hypothalamus including both medial and lateral divisions ( AH , MAH , LAH ) .
	manualset3
209217	6	418128	7	NULL	NULL	0	NULL	 regions 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	With stereotaxic methods under chloralose anesthesia the hypothalami of naturally estrous or estrogen-gonadotropin-primed queens were stimulated bilaterally in one of the following regions : medial basal hypothalamus including the premamillary area ( MBH ) and the anterior hypothalamus including both medial and lateral divisions ( AH , MAH , LAH ) .
	manualset3
209218	7	418128	7	NULL	NULL	0	NULL	medial basal hypothalamus including the premamillary area ( MBH )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	With stereotaxic methods under chloralose anesthesia the hypothalami of naturally estrous or estrogen-gonadotropin-primed queens were stimulated bilaterally in one of the following regions : medial basal hypothalamus including the premamillary area ( MBH ) and the anterior hypothalamus including both medial and lateral divisions ( AH , MAH , LAH ) .
	manualset3
209219	8	418128	7	NULL	NULL	0	NULL	anterior hypothalamus including both medial and lateral divisions ( AH , MAH , LAH )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	With stereotaxic methods under chloralose anesthesia the hypothalami of naturally estrous or estrogen-gonadotropin-primed queens were stimulated bilaterally in one of the following regions : medial basal hypothalamus including the premamillary area ( MBH ) and the anterior hypothalamus including both medial and lateral divisions ( AH , MAH , LAH ) .
	manualset3
209220	1	418129	7	NULL	NULL	0	NULL	enumerative stepwise ansatz	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An enumerative stepwise ansatz enables atomic-accuracy RNA loop modeling .
	manualset3
209221	2	418129	7	NULL	NULL	0	NULL	atomic-accuracy RNA loop modeling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An enumerative stepwise ansatz enables atomic-accuracy RNA loop modeling .
	manualset3
209222	1	418130	7	NULL	NULL	0	NULL	Unfixed cryostat sections	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfixed cryostat sections from 4 animals per month of pregnancy and 5 animals per peripartal group ( in total 51 pregnancies ) were used to immunolocalize collagen types I , III , and IV by an indirect FITC method .
	manualset3
209223	2	418130	7	NULL	NULL	NULL	NULL	 4 animals per month	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Unfixed cryostat sections from 4 animals per month of pregnancy and 5 animals per peripartal group ( in total 51 pregnancies ) were used to immunolocalize collagen types I , III , and IV by an indirect FITC method .
	manualset3
209224	3	418130	7	NULL	NULL	0	NULL	 pregnancy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfixed cryostat sections from 4 animals per month of pregnancy and 5 animals per peripartal group ( in total 51 pregnancies ) were used to immunolocalize collagen types I , III , and IV by an indirect FITC method .
	manualset3
209225	4	418130	7	NULL	NULL	0	NULL	5 animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfixed cryostat sections from 4 animals per month of pregnancy and 5 animals per peripartal group ( in total 51 pregnancies ) were used to immunolocalize collagen types I , III , and IV by an indirect FITC method .
	manualset3
209226	5	418130	7	NULL	NULL	0	NULL	peripartal group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfixed cryostat sections from 4 animals per month of pregnancy and 5 animals per peripartal group ( in total 51 pregnancies ) were used to immunolocalize collagen types I , III , and IV by an indirect FITC method .
	manualset3
209227	6	418130	7	NULL	NULL	0	NULL	collagen types I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfixed cryostat sections from 4 animals per month of pregnancy and 5 animals per peripartal group ( in total 51 pregnancies ) were used to immunolocalize collagen types I , III , and IV by an indirect FITC method .
	manualset3
209228	7	418130	7	NULL	NULL	0	NULL	collagen types III	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfixed cryostat sections from 4 animals per month of pregnancy and 5 animals per peripartal group ( in total 51 pregnancies ) were used to immunolocalize collagen types I , III , and IV by an indirect FITC method .
	manualset3
209229	8	418130	7	NULL	NULL	0	NULL	collagen types IV	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfixed cryostat sections from 4 animals per month of pregnancy and 5 animals per peripartal group ( in total 51 pregnancies ) were used to immunolocalize collagen types I , III , and IV by an indirect FITC method .
	manualset3
209230	9	418130	7	NULL	NULL	0	NULL	indirect FITC method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfixed cryostat sections from 4 animals per month of pregnancy and 5 animals per peripartal group ( in total 51 pregnancies ) were used to immunolocalize collagen types I , III , and IV by an indirect FITC method .
	manualset3
209231	10	418130	7	NULL	NULL	0	NULL	 total 51 pregnancies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfixed cryostat sections from 4 animals per month of pregnancy and 5 animals per peripartal group ( in total 51 pregnancies ) were used to immunolocalize collagen types I , III , and IV by an indirect FITC method .
	manualset3
209235	1	418131	7	NULL	NULL	0	NULL	3 , 5-bis - ( pyridin-4-yl-methyl-amino ) - benzoate anion	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Each 3 , 5-bis - ( pyridin-4-yl-methyl-amino ) - benzoate anion acts as a ( 2 ) - bridge , linking different nickel ions into a chain along ( 010 ) .
	manualset3
209236	2	418131	7	NULL	NULL	0	NULL	( 2 ) - bridge 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Each 3 , 5-bis - ( pyridin-4-yl-methyl-amino ) - benzoate anion acts as a ( 2 ) - bridge , linking different nickel ions into a chain along ( 010 ) .
	manualset3
209237	3	418131	7	NULL	NULL	0	NULL	nickel ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Each 3 , 5-bis - ( pyridin-4-yl-methyl-amino ) - benzoate anion acts as a ( 2 ) - bridge , linking different nickel ions into a chain along ( 010 ) .
	manualset3
209238	4	418131	7	NULL	NULL	0	NULL	chain	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Each 3 , 5-bis - ( pyridin-4-yl-methyl-amino ) - benzoate anion acts as a ( 2 ) - bridge , linking different nickel ions into a chain along ( 010 ) .
	manualset3
209239	1	418132	7	NULL	NULL	0	NULL	Enhancing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Enhancing consumer independence through delegation .
	manualset3
209240	2	418132	7	NULL	NULL	0	NULL	delegation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Enhancing consumer independence through delegation .
	manualset3
209241	1	418133	7	NULL	NULL	0	NULL	Fusion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fusion of such erythrocytes results in formation of giant cells up to 130 microm in diameter .
	manualset3
209242	2	418133	7	NULL	NULL	0	NULL	erythrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Fusion of such erythrocytes results in formation of giant cells up to 130 microm in diameter .
	manualset3
209243	3	418133	7	NULL	NULL	0	NULL	 formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fusion of such erythrocytes results in formation of giant cells up to 130 microm in diameter .
	manualset3
209244	4	418133	7	NULL	NULL	0	NULL	giant cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Fusion of such erythrocytes results in formation of giant cells up to 130 microm in diameter .
	manualset3
209245	5	418133	7	NULL	NULL	0	NULL	130 microm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Fusion of such erythrocytes results in formation of giant cells up to 130 microm in diameter .
	manualset3
209246	6	418133	7	NULL	NULL	0	NULL	diameter	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Fusion of such erythrocytes results in formation of giant cells up to 130 microm in diameter .
	manualset3
209247	1	418134	7	NULL	NULL	0	NULL	anti-proteinase IgG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean anti-proteinase IgG stabilized at high titer by week 5 post-infection , while IgM titers decreased to near background levels .
	manualset3
209248	2	418134	7	NULL	NULL	0	NULL	high titer 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean anti-proteinase IgG stabilized at high titer by week 5 post-infection , while IgM titers decreased to near background levels .
	manualset3
209249	3	418134	7	NULL	NULL	NULL	NULL	post-infection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mean anti-proteinase IgG stabilized at high titer by week 5 post-infection , while IgM titers decreased to near background levels .
	manualset3
209250	4	418134	7	NULL	NULL	0	NULL	IgM titers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean anti-proteinase IgG stabilized at high titer by week 5 post-infection , while IgM titers decreased to near background levels .
	manualset3
209251	5	418134	7	NULL	NULL	0	NULL	background levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean anti-proteinase IgG stabilized at high titer by week 5 post-infection , while IgM titers decreased to near background levels .
	manualset3
209252	6	418134	7	NULL	NULL	0	NULL	week 5	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean anti-proteinase IgG stabilized at high titer by week 5 post-infection , while IgM titers decreased to near background levels .
	manualset3
209253	1	418135	7	NULL	NULL	0	NULL	Allele-specific mismatch amplification mutation assays ( MAMA )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Allele-specific mismatch amplification mutation assays ( MAMA ) of anatomically distinct sectors of the upper bronchial tracts of nine nonsmokers revealed many numerically dispersed clusters of the point mutations C742T , G746T , G747T of the TP53 gene , G35T of the KRAS gene and G508A of the HPRT1 gene .
	manualset3
209254	2	418135	7	NULL	NULL	0	NULL	anatomically distinct sectors 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Allele-specific mismatch amplification mutation assays ( MAMA ) of anatomically distinct sectors of the upper bronchial tracts of nine nonsmokers revealed many numerically dispersed clusters of the point mutations C742T , G746T , G747T of the TP53 gene , G35T of the KRAS gene and G508A of the HPRT1 gene .
	manualset3
209255	3	418135	7	NULL	NULL	0	NULL	upper bronchial tracts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Allele-specific mismatch amplification mutation assays ( MAMA ) of anatomically distinct sectors of the upper bronchial tracts of nine nonsmokers revealed many numerically dispersed clusters of the point mutations C742T , G746T , G747T of the TP53 gene , G35T of the KRAS gene and G508A of the HPRT1 gene .
	manualset3
209256	4	418135	7	NULL	NULL	0	NULL	nine nonsmokers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Allele-specific mismatch amplification mutation assays ( MAMA ) of anatomically distinct sectors of the upper bronchial tracts of nine nonsmokers revealed many numerically dispersed clusters of the point mutations C742T , G746T , G747T of the TP53 gene , G35T of the KRAS gene and G508A of the HPRT1 gene .
	manualset3
209257	5	418135	7	NULL	NULL	0	NULL	dispersed clusters	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Allele-specific mismatch amplification mutation assays ( MAMA ) of anatomically distinct sectors of the upper bronchial tracts of nine nonsmokers revealed many numerically dispersed clusters of the point mutations C742T , G746T , G747T of the TP53 gene , G35T of the KRAS gene and G508A of the HPRT1 gene .
	manualset3
209258	6	418135	7	NULL	NULL	0	NULL	point mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Allele-specific mismatch amplification mutation assays ( MAMA ) of anatomically distinct sectors of the upper bronchial tracts of nine nonsmokers revealed many numerically dispersed clusters of the point mutations C742T , G746T , G747T of the TP53 gene , G35T of the KRAS gene and G508A of the HPRT1 gene .
	manualset3
209259	7	418135	7	NULL	NULL	NULL	NULL	C742T	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Allele-specific mismatch amplification mutation assays ( MAMA ) of anatomically distinct sectors of the upper bronchial tracts of nine nonsmokers revealed many numerically dispersed clusters of the point mutations C742T , G746T , G747T of the TP53 gene , G35T of the KRAS gene and G508A of the HPRT1 gene .
	manualset3
209260	8	418135	7	NULL	NULL	0	NULL	G746T	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Allele-specific mismatch amplification mutation assays ( MAMA ) of anatomically distinct sectors of the upper bronchial tracts of nine nonsmokers revealed many numerically dispersed clusters of the point mutations C742T , G746T , G747T of the TP53 gene , G35T of the KRAS gene and G508A of the HPRT1 gene .
	manualset3
209261	9	418135	7	NULL	NULL	0	NULL	 G747T	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Allele-specific mismatch amplification mutation assays ( MAMA ) of anatomically distinct sectors of the upper bronchial tracts of nine nonsmokers revealed many numerically dispersed clusters of the point mutations C742T , G746T , G747T of the TP53 gene , G35T of the KRAS gene and G508A of the HPRT1 gene .
	manualset3
209262	10	418135	7	NULL	NULL	0	NULL	TP53 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Allele-specific mismatch amplification mutation assays ( MAMA ) of anatomically distinct sectors of the upper bronchial tracts of nine nonsmokers revealed many numerically dispersed clusters of the point mutations C742T , G746T , G747T of the TP53 gene , G35T of the KRAS gene and G508A of the HPRT1 gene .
	manualset3
209263	11	418135	7	NULL	NULL	0	NULL	G35T	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Allele-specific mismatch amplification mutation assays ( MAMA ) of anatomically distinct sectors of the upper bronchial tracts of nine nonsmokers revealed many numerically dispersed clusters of the point mutations C742T , G746T , G747T of the TP53 gene , G35T of the KRAS gene and G508A of the HPRT1 gene .
	manualset3
209264	12	418135	7	NULL	NULL	0	NULL	KRAS gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Allele-specific mismatch amplification mutation assays ( MAMA ) of anatomically distinct sectors of the upper bronchial tracts of nine nonsmokers revealed many numerically dispersed clusters of the point mutations C742T , G746T , G747T of the TP53 gene , G35T of the KRAS gene and G508A of the HPRT1 gene .
	manualset3
209265	13	418135	7	NULL	NULL	0	NULL	G508A	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Allele-specific mismatch amplification mutation assays ( MAMA ) of anatomically distinct sectors of the upper bronchial tracts of nine nonsmokers revealed many numerically dispersed clusters of the point mutations C742T , G746T , G747T of the TP53 gene , G35T of the KRAS gene and G508A of the HPRT1 gene .
	manualset3
209266	14	418135	7	NULL	NULL	0	NULL	HPRT1 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Allele-specific mismatch amplification mutation assays ( MAMA ) of anatomically distinct sectors of the upper bronchial tracts of nine nonsmokers revealed many numerically dispersed clusters of the point mutations C742T , G746T , G747T of the TP53 gene , G35T of the KRAS gene and G508A of the HPRT1 gene .
	manualset3
209267	1	418136	7	NULL	NULL	0	NULL	45 stacked strain gauge rosettes	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Three 45 stacked strain gauge rosettes were affixed along the length of the radius quantifying the bone strains .
	manualset3
209268	2	418136	7	NULL	NULL	0	NULL	 length	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Three 45 stacked strain gauge rosettes were affixed along the length of the radius quantifying the bone strains .
	manualset3
209269	3	418136	7	NULL	NULL	0	NULL	 radius	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Three 45 stacked strain gauge rosettes were affixed along the length of the radius quantifying the bone strains .
	manualset3
209270	4	418136	7	NULL	NULL	NULL	NULL	bone strains	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Three 45 stacked strain gauge rosettes were affixed along the length of the radius quantifying the bone strains .
	manualset3
209271	1	418137	7	NULL	NULL	0	NULL	Bilateral atrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Bilateral atrophy of the frontal and temporal lobes in schizophrenic patients with Capgras syndrome : a case-control study using computed tomography .
	manualset3
209272	2	418137	7	NULL	NULL	0	NULL	 frontal lobes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Bilateral atrophy of the frontal and temporal lobes in schizophrenic patients with Capgras syndrome : a case-control study using computed tomography .
	manualset3
209273	3	418137	7	NULL	NULL	0	NULL	 temporal lobes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Bilateral atrophy of the frontal and temporal lobes in schizophrenic patients with Capgras syndrome : a case-control study using computed tomography .
	manualset3
209274	4	418137	7	NULL	NULL	0	NULL	schizophrenic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Bilateral atrophy of the frontal and temporal lobes in schizophrenic patients with Capgras syndrome : a case-control study using computed tomography .
	manualset3
209275	5	418137	7	NULL	NULL	0	NULL	Capgras syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Bilateral atrophy of the frontal and temporal lobes in schizophrenic patients with Capgras syndrome : a case-control study using computed tomography .
	manualset3
209276	6	418137	7	NULL	NULL	NULL	NULL	case-control study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bilateral atrophy of the frontal and temporal lobes in schizophrenic patients with Capgras syndrome : a case-control study using computed tomography .
	manualset3
209277	7	418137	7	NULL	NULL	0	NULL	 computed tomography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Bilateral atrophy of the frontal and temporal lobes in schizophrenic patients with Capgras syndrome : a case-control study using computed tomography .
	manualset3
209278	1	418138	7	NULL	NULL	0	NULL	Analytical results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Analytical results can be obtained in the limit alpha -- ) infinity and , for large alpha , by perturbation expansion .
	manualset3
209279	2	418138	7	NULL	NULL	0	NULL	alpha -- ) infinity	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Analytical results can be obtained in the limit alpha -- ) infinity and , for large alpha , by perturbation expansion .
	manualset3
209280	3	418138	7	NULL	NULL	0	NULL	large alpha	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Analytical results can be obtained in the limit alpha -- ) infinity and , for large alpha , by perturbation expansion .
	manualset3
209281	4	418138	7	NULL	NULL	0	NULL	perturbation expansion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Analytical results can be obtained in the limit alpha -- ) infinity and , for large alpha , by perturbation expansion .
	manualset3
209282	1	418139	7	NULL	NULL	0	NULL	ANP	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	ANP caused a slight but significant enhancement of vasopressin-stimulated IP3 production , but had no effect on the cytosolic calcium response nor on the contractile response .
	manualset3
209283	2	418139	7	NULL	NULL	0	NULL	enhancement	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	ANP caused a slight but significant enhancement of vasopressin-stimulated IP3 production , but had no effect on the cytosolic calcium response nor on the contractile response .
	manualset3
209284	3	418139	7	NULL	NULL	0	NULL	vasopressin-stimulated IP3 production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	ANP caused a slight but significant enhancement of vasopressin-stimulated IP3 production , but had no effect on the cytosolic calcium response nor on the contractile response .
	manualset3
209285	4	418139	7	NULL	NULL	0	NULL	no effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	ANP caused a slight but significant enhancement of vasopressin-stimulated IP3 production , but had no effect on the cytosolic calcium response nor on the contractile response .
	manualset3
209286	5	418139	7	NULL	NULL	0	NULL	cytosolic calcium response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	ANP caused a slight but significant enhancement of vasopressin-stimulated IP3 production , but had no effect on the cytosolic calcium response nor on the contractile response .
	manualset3
209287	6	418139	7	NULL	NULL	0	NULL	contractile response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	ANP caused a slight but significant enhancement of vasopressin-stimulated IP3 production , but had no effect on the cytosolic calcium response nor on the contractile response .
	manualset3
209288	1	418140	7	NULL	NULL	0	NULL	day 1	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 1 after injury the intensity of astrocyte proliferation showed dose-dependent changes .
	manualset3
209289	2	418140	7	NULL	NULL	0	NULL	 injury 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 1 after injury the intensity of astrocyte proliferation showed dose-dependent changes .
	manualset3
209290	3	418140	7	NULL	NULL	0	NULL	 intensity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 1 after injury the intensity of astrocyte proliferation showed dose-dependent changes .
	manualset3
209291	4	418140	7	NULL	NULL	0	NULL	astrocyte proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 1 after injury the intensity of astrocyte proliferation showed dose-dependent changes .
	manualset3
209292	5	418140	7	NULL	NULL	0	NULL	dose-dependent changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On day 1 after injury the intensity of astrocyte proliferation showed dose-dependent changes .
	manualset3
209293	1	418141	7	NULL	NULL	0	NULL	Survival outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Survival outcomes in resected extrahepatic cholangiocarcinoma : effect of adjuvant radiotherapy in a surveillance , epidemiology , and end results analysis .
	manualset3
209294	2	418141	7	NULL	NULL	0	NULL	resected extrahepatic cholangiocarcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Survival outcomes in resected extrahepatic cholangiocarcinoma : effect of adjuvant radiotherapy in a surveillance , epidemiology , and end results analysis .
	manualset3
209295	3	418141	7	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Survival outcomes in resected extrahepatic cholangiocarcinoma : effect of adjuvant radiotherapy in a surveillance , epidemiology , and end results analysis .
	manualset3
209296	4	418141	7	NULL	NULL	0	NULL	adjuvant radiotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Survival outcomes in resected extrahepatic cholangiocarcinoma : effect of adjuvant radiotherapy in a surveillance , epidemiology , and end results analysis .
	manualset3
209297	5	418141	7	NULL	NULL	0	NULL	surveillance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Survival outcomes in resected extrahepatic cholangiocarcinoma : effect of adjuvant radiotherapy in a surveillance , epidemiology , and end results analysis .
	manualset3
209298	6	418141	7	NULL	NULL	0	NULL	epidemiology 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Survival outcomes in resected extrahepatic cholangiocarcinoma : effect of adjuvant radiotherapy in a surveillance , epidemiology , and end results analysis .
	manualset3
209299	7	418141	7	NULL	NULL	0	NULL	end results analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Survival outcomes in resected extrahepatic cholangiocarcinoma : effect of adjuvant radiotherapy in a surveillance , epidemiology , and end results analysis .
	manualset3
209300	1	418142	7	NULL	NULL	NULL	NULL	Labeling mitochondria	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Labeling mitochondria with TMRM or TMRE .
	manualset3
209301	2	418142	7	NULL	NULL	0	NULL	TMRM	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Labeling mitochondria with TMRM or TMRE .
	manualset3
209302	3	418142	7	NULL	NULL	0	NULL	TMRE	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Labeling mitochondria with TMRM or TMRE .
	manualset3
209303	1	418143	7	NULL	NULL	0	NULL	Elimination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Elimination of potassium in rabbits with kidneys reduced surgically ) .
	manualset3
209304	2	418143	7	NULL	NULL	0	NULL	potassium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Elimination of potassium in rabbits with kidneys reduced surgically ) .
	manualset3
209305	3	418143	7	NULL	NULL	0	NULL	 rabbits	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Elimination of potassium in rabbits with kidneys reduced surgically ) .
	manualset3
209306	4	418143	7	NULL	NULL	NULL	NULL	kidneys reduced surgically	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Elimination of potassium in rabbits with kidneys reduced surgically ) .
	manualset3
209307	1	418144	7	NULL	NULL	0	NULL	Allele frequencies	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Allele frequencies and sequence characteristics of D2S1242 STR locus in Chinese population .
	manualset3
209308	2	418144	7	NULL	NULL	0	NULL	sequence characteristics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Allele frequencies and sequence characteristics of D2S1242 STR locus in Chinese population .
	manualset3
209309	3	418144	7	NULL	NULL	0	NULL	D2S1242 STR locus	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Allele frequencies and sequence characteristics of D2S1242 STR locus in Chinese population .
	manualset3
209310	4	418144	7	NULL	NULL	0	NULL	Chinese population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Allele frequencies and sequence characteristics of D2S1242 STR locus in Chinese population .
	manualset3
209311	1	418145	7	NULL	NULL	0	NULL	Effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of vegetation types on soil respiration characteristics on a smaller scale ) .
	manualset3
209312	2	418145	7	NULL	NULL	NULL	NULL	vegetation types 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Effect of vegetation types on soil respiration characteristics on a smaller scale ) .
	manualset3
209313	3	418145	7	NULL	NULL	0	NULL	soil respiration characteristics	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of vegetation types on soil respiration characteristics on a smaller scale ) .
	manualset3
209314	4	418145	7	NULL	NULL	0	NULL	smaller scale 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of vegetation types on soil respiration characteristics on a smaller scale ) .
	manualset3
209315	1	418146	7	NULL	NULL	0	NULL	 rate of proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of proliferation was determined by immunocytochemical detection of BrdU-incorporating cells located next to or far from the wound .
	manualset3
209316	2	418146	7	NULL	NULL	0	NULL	immunocytochemical detection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of proliferation was determined by immunocytochemical detection of BrdU-incorporating cells located next to or far from the wound .
	manualset3
209317	3	418146	7	NULL	NULL	0	NULL	BrdU-incorporating cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of proliferation was determined by immunocytochemical detection of BrdU-incorporating cells located next to or far from the wound .
	manualset3
209318	4	418146	7	NULL	NULL	0	NULL	wound	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of proliferation was determined by immunocytochemical detection of BrdU-incorporating cells located next to or far from the wound .
	manualset3
209319	1	418147	7	NULL	NULL	0	NULL	4-5 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	For 4-5 weeks after CBL , cirrhotic rats showed sodium retention relative to control rats without any sign of ascites .
	manualset3
209320	2	418147	7	NULL	NULL	0	NULL	CBL	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For 4-5 weeks after CBL , cirrhotic rats showed sodium retention relative to control rats without any sign of ascites .
	manualset3
209321	3	418147	7	NULL	NULL	0	NULL	cirrhotic rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For 4-5 weeks after CBL , cirrhotic rats showed sodium retention relative to control rats without any sign of ascites .
	manualset3
209322	4	418147	7	NULL	NULL	0	NULL	sodium retention	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For 4-5 weeks after CBL , cirrhotic rats showed sodium retention relative to control rats without any sign of ascites .
	manualset3
209323	5	418147	7	NULL	NULL	0	NULL	control rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For 4-5 weeks after CBL , cirrhotic rats showed sodium retention relative to control rats without any sign of ascites .
	manualset3
209324	6	418147	7	NULL	NULL	0	NULL	sign of ascites	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For 4-5 weeks after CBL , cirrhotic rats showed sodium retention relative to control rats without any sign of ascites .
	manualset3
209325	1	418148	7	NULL	NULL	0	NULL	adverse trends	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Both adverse trends have been shown to be associated with year of birth .
	manualset3
209326	2	418148	7	NULL	NULL	0	NULL	year of birth	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Both adverse trends have been shown to be associated with year of birth .
	manualset3
209327	1	418149	7	NULL	NULL	0	NULL	Cystic fibrosis ( CF )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Cystic fibrosis ( CF ) , the most common lethal genetic disease in Caucasians , is characterized by defective electrolyte transport in several epithelia .
	manualset3
209328	2	418149	7	NULL	NULL	0	NULL	 lethal genetic disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Cystic fibrosis ( CF ) , the most common lethal genetic disease in Caucasians , is characterized by defective electrolyte transport in several epithelia .
	manualset3
209329	3	418149	7	NULL	NULL	0	NULL	Caucasians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Cystic fibrosis ( CF ) , the most common lethal genetic disease in Caucasians , is characterized by defective electrolyte transport in several epithelia .
	manualset3
209330	4	418149	7	NULL	NULL	0	NULL	defective electrolyte transport	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cystic fibrosis ( CF ) , the most common lethal genetic disease in Caucasians , is characterized by defective electrolyte transport in several epithelia .
	manualset3
209331	5	418149	7	NULL	NULL	0	NULL	several epithelia	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Cystic fibrosis ( CF ) , the most common lethal genetic disease in Caucasians , is characterized by defective electrolyte transport in several epithelia .
	manualset3
209332	1	418150	7	NULL	NULL	NULL	NULL	Natural history	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Natural history of contractile abnormalities after acute myocardial infarction in man : severity and response to nitroglycerin as a function of time .
	manualset3
209333	2	418150	7	NULL	NULL	0	NULL	contractile abnormalities 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural history of contractile abnormalities after acute myocardial infarction in man : severity and response to nitroglycerin as a function of time .
	manualset3
209334	3	418150	7	NULL	NULL	0	NULL	acute myocardial infarction	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural history of contractile abnormalities after acute myocardial infarction in man : severity and response to nitroglycerin as a function of time .
	manualset3
209335	4	418150	7	NULL	NULL	0	NULL	man	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural history of contractile abnormalities after acute myocardial infarction in man : severity and response to nitroglycerin as a function of time .
	manualset3
209336	5	418150	7	NULL	NULL	0	NULL	severity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural history of contractile abnormalities after acute myocardial infarction in man : severity and response to nitroglycerin as a function of time .
	manualset3
209337	6	418150	7	NULL	NULL	0	NULL	response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural history of contractile abnormalities after acute myocardial infarction in man : severity and response to nitroglycerin as a function of time .
	manualset3
209338	7	418150	7	NULL	NULL	0	NULL	nitroglycerin 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural history of contractile abnormalities after acute myocardial infarction in man : severity and response to nitroglycerin as a function of time .
	manualset3
209339	8	418150	7	NULL	NULL	0	NULL	 function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural history of contractile abnormalities after acute myocardial infarction in man : severity and response to nitroglycerin as a function of time .
	manualset3
209340	9	418150	7	NULL	NULL	0	NULL	 time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural history of contractile abnormalities after acute myocardial infarction in man : severity and response to nitroglycerin as a function of time .
	manualset3
209341	1	418151	7	NULL	NULL	0	NULL	countries	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Several countries have discussed how to treat burn victims , but only a little is known of their capacity to offer space to other countries in the event of a fire disaster outside the country in question .
	manualset3
209342	2	418151	7	NULL	NULL	NULL	NULL	burn victims	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Several countries have discussed how to treat burn victims , but only a little is known of their capacity to offer space to other countries in the event of a fire disaster outside the country in question .
	manualset3
209343	3	418151	7	NULL	NULL	NULL	NULL	 space	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Several countries have discussed how to treat burn victims , but only a little is known of their capacity to offer space to other countries in the event of a fire disaster outside the country in question .
	manualset3
209344	4	418151	7	NULL	NULL	0	NULL	countries	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Several countries have discussed how to treat burn victims , but only a little is known of their capacity to offer space to other countries in the event of a fire disaster outside the country in question .
	manualset3
209345	5	418151	7	NULL	NULL	0	NULL	 event 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Several countries have discussed how to treat burn victims , but only a little is known of their capacity to offer space to other countries in the event of a fire disaster outside the country in question .
	manualset3
209346	6	418151	7	NULL	NULL	0	NULL	fire disaster	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several countries have discussed how to treat burn victims , but only a little is known of their capacity to offer space to other countries in the event of a fire disaster outside the country in question .
	manualset3
209347	7	418151	7	NULL	NULL	0	NULL	country	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Several countries have discussed how to treat burn victims , but only a little is known of their capacity to offer space to other countries in the event of a fire disaster outside the country in question .
	manualset3
209348	8	418151	7	NULL	NULL	0	NULL	question	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Several countries have discussed how to treat burn victims , but only a little is known of their capacity to offer space to other countries in the event of a fire disaster outside the country in question .
	manualset3
209349	9	418151	7	NULL	NULL	0	NULL	capacity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several countries have discussed how to treat burn victims , but only a little is known of their capacity to offer space to other countries in the event of a fire disaster outside the country in question .
	manualset3
209350	1	418152	7	NULL	NULL	NULL	NULL	 electrophysiological experiment	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the present electrophysiological experiment , the percentage of DRG neurons that responded to alpha ( beta ) meATP with slow desensitizing inward current remained constant in capsaicin-treated rats , whereas the percentage that responded with rapid desensitizing current dramatically decreased .
	manualset3
209351	2	418152	7	NULL	NULL	0	NULL	percentage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present electrophysiological experiment , the percentage of DRG neurons that responded to alpha ( beta ) meATP with slow desensitizing inward current remained constant in capsaicin-treated rats , whereas the percentage that responded with rapid desensitizing current dramatically decreased .
	manualset3
209352	3	418152	7	NULL	NULL	0	NULL	DRG neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present electrophysiological experiment , the percentage of DRG neurons that responded to alpha ( beta ) meATP with slow desensitizing inward current remained constant in capsaicin-treated rats , whereas the percentage that responded with rapid desensitizing current dramatically decreased .
	manualset3
209353	4	418152	7	NULL	NULL	0	NULL	alpha ( beta ) meATP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present electrophysiological experiment , the percentage of DRG neurons that responded to alpha ( beta ) meATP with slow desensitizing inward current remained constant in capsaicin-treated rats , whereas the percentage that responded with rapid desensitizing current dramatically decreased .
	manualset3
209354	5	418152	7	NULL	NULL	0	NULL	slow desensitizing inward current	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present electrophysiological experiment , the percentage of DRG neurons that responded to alpha ( beta ) meATP with slow desensitizing inward current remained constant in capsaicin-treated rats , whereas the percentage that responded with rapid desensitizing current dramatically decreased .
	manualset3
209355	6	418152	7	NULL	NULL	0	NULL	capsaicin-treated rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present electrophysiological experiment , the percentage of DRG neurons that responded to alpha ( beta ) meATP with slow desensitizing inward current remained constant in capsaicin-treated rats , whereas the percentage that responded with rapid desensitizing current dramatically decreased .
	manualset3
209356	7	418152	7	NULL	NULL	0	NULL	percentage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present electrophysiological experiment , the percentage of DRG neurons that responded to alpha ( beta ) meATP with slow desensitizing inward current remained constant in capsaicin-treated rats , whereas the percentage that responded with rapid desensitizing current dramatically decreased .
	manualset3
209357	8	418152	7	NULL	NULL	0	NULL	rapid desensitizing current	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present electrophysiological experiment , the percentage of DRG neurons that responded to alpha ( beta ) meATP with slow desensitizing inward current remained constant in capsaicin-treated rats , whereas the percentage that responded with rapid desensitizing current dramatically decreased .
	manualset3
209358	1	418153	7	NULL	NULL	0	NULL	Expressions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Expressions of TNF-alpha and IL-1beta in human ischemic brain tissues ) .
	manualset3
209359	2	418153	7	NULL	NULL	0	NULL	TNF-alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Expressions of TNF-alpha and IL-1beta in human ischemic brain tissues ) .
	manualset3
209360	3	418153	7	NULL	NULL	0	NULL	IL-1beta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Expressions of TNF-alpha and IL-1beta in human ischemic brain tissues ) .
	manualset3
209361	4	418153	7	NULL	NULL	0	NULL	human ischemic brain tissues 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	( Expressions of TNF-alpha and IL-1beta in human ischemic brain tissues ) .
	manualset3
209362	1	418154	7	NULL	NULL	0	NULL	Ultrasonography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasonography and conventional radiography was utilized to make the diagnosis and to plan and perform puncture and drainage .
	manualset3
209363	2	418154	7	NULL	NULL	0	NULL	conventional radiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasonography and conventional radiography was utilized to make the diagnosis and to plan and perform puncture and drainage .
	manualset3
209364	3	418154	7	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasonography and conventional radiography was utilized to make the diagnosis and to plan and perform puncture and drainage .
	manualset3
209365	4	418154	7	NULL	NULL	0	NULL	puncture	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasonography and conventional radiography was utilized to make the diagnosis and to plan and perform puncture and drainage .
	manualset3
209366	5	418154	7	NULL	NULL	0	NULL	 drainage	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasonography and conventional radiography was utilized to make the diagnosis and to plan and perform puncture and drainage .
	manualset3
209367	1	418155	7	NULL	NULL	0	NULL	novel hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel hypothesis for the development of chronic pain states that a strong nociceptive input to the spinal cord leads to cell death predominantly in inhibitory interneurones .
	manualset3
209368	2	418155	7	NULL	NULL	0	NULL	development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel hypothesis for the development of chronic pain states that a strong nociceptive input to the spinal cord leads to cell death predominantly in inhibitory interneurones .
	manualset3
209369	3	418155	7	NULL	NULL	0	NULL	chronic pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel hypothesis for the development of chronic pain states that a strong nociceptive input to the spinal cord leads to cell death predominantly in inhibitory interneurones .
	manualset3
209370	4	418155	7	NULL	NULL	NULL	NULL	strong nociceptive input	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A novel hypothesis for the development of chronic pain states that a strong nociceptive input to the spinal cord leads to cell death predominantly in inhibitory interneurones .
	manualset3
209371	5	418155	7	NULL	NULL	0	NULL	spinal cord	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel hypothesis for the development of chronic pain states that a strong nociceptive input to the spinal cord leads to cell death predominantly in inhibitory interneurones .
	manualset3
209372	6	418155	7	NULL	NULL	0	NULL	cell death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel hypothesis for the development of chronic pain states that a strong nociceptive input to the spinal cord leads to cell death predominantly in inhibitory interneurones .
	manualset3
209373	7	418155	7	NULL	NULL	0	NULL	inhibitory interneurones	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel hypothesis for the development of chronic pain states that a strong nociceptive input to the spinal cord leads to cell death predominantly in inhibitory interneurones .
	manualset3
209374	1	418156	7	NULL	NULL	0	NULL	 incidence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of the structural features on the self-assembly of different poloxamines ( the conventional sequential Tetronic 304 , 901 , 904 , 908 , 1107 , 1301 , and 1307 ; a reverse-sequential counterpart Tetronic 150R1 ; and a chemically modified derivative , N-methylated Tetronic 1107 ) was thoroughly studied in 10 mM HCl by means of pi-A isotherm , surface tension , and pyrene fluorescence measurements .
	manualset3
209375	2	418156	7	NULL	NULL	0	NULL	structural features	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of the structural features on the self-assembly of different poloxamines ( the conventional sequential Tetronic 304 , 901 , 904 , 908 , 1107 , 1301 , and 1307 ; a reverse-sequential counterpart Tetronic 150R1 ; and a chemically modified derivative , N-methylated Tetronic 1107 ) was thoroughly studied in 10 mM HCl by means of pi-A isotherm , surface tension , and pyrene fluorescence measurements .
	manualset3
209376	3	418156	7	NULL	NULL	0	NULL	self-assembly	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of the structural features on the self-assembly of different poloxamines ( the conventional sequential Tetronic 304 , 901 , 904 , 908 , 1107 , 1301 , and 1307 ; a reverse-sequential counterpart Tetronic 150R1 ; and a chemically modified derivative , N-methylated Tetronic 1107 ) was thoroughly studied in 10 mM HCl by means of pi-A isotherm , surface tension , and pyrene fluorescence measurements .
	manualset3
209377	4	418156	7	NULL	NULL	0	NULL	poloxamines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of the structural features on the self-assembly of different poloxamines ( the conventional sequential Tetronic 304 , 901 , 904 , 908 , 1107 , 1301 , and 1307 ; a reverse-sequential counterpart Tetronic 150R1 ; and a chemically modified derivative , N-methylated Tetronic 1107 ) was thoroughly studied in 10 mM HCl by means of pi-A isotherm , surface tension , and pyrene fluorescence measurements .
	manualset3
209378	5	418156	7	NULL	NULL	0	NULL	conventional sequential Tetronic 304	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of the structural features on the self-assembly of different poloxamines ( the conventional sequential Tetronic 304 , 901 , 904 , 908 , 1107 , 1301 , and 1307 ; a reverse-sequential counterpart Tetronic 150R1 ; and a chemically modified derivative , N-methylated Tetronic 1107 ) was thoroughly studied in 10 mM HCl by means of pi-A isotherm , surface tension , and pyrene fluorescence measurements .
	manualset3
209379	6	418156	7	NULL	NULL	0	NULL	conventional sequential Tetronic 901	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of the structural features on the self-assembly of different poloxamines ( the conventional sequential Tetronic 304 , 901 , 904 , 908 , 1107 , 1301 , and 1307 ; a reverse-sequential counterpart Tetronic 150R1 ; and a chemically modified derivative , N-methylated Tetronic 1107 ) was thoroughly studied in 10 mM HCl by means of pi-A isotherm , surface tension , and pyrene fluorescence measurements .
	manualset3
209380	7	418156	7	NULL	NULL	0	NULL	conventional sequential Tetronic 904	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of the structural features on the self-assembly of different poloxamines ( the conventional sequential Tetronic 304 , 901 , 904 , 908 , 1107 , 1301 , and 1307 ; a reverse-sequential counterpart Tetronic 150R1 ; and a chemically modified derivative , N-methylated Tetronic 1107 ) was thoroughly studied in 10 mM HCl by means of pi-A isotherm , surface tension , and pyrene fluorescence measurements .
	manualset3
209381	8	418156	7	NULL	NULL	0	NULL	conventional sequential Tetronic 908	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of the structural features on the self-assembly of different poloxamines ( the conventional sequential Tetronic 304 , 901 , 904 , 908 , 1107 , 1301 , and 1307 ; a reverse-sequential counterpart Tetronic 150R1 ; and a chemically modified derivative , N-methylated Tetronic 1107 ) was thoroughly studied in 10 mM HCl by means of pi-A isotherm , surface tension , and pyrene fluorescence measurements .
	manualset3
209382	9	418156	7	NULL	NULL	0	NULL	conventional sequential Tetronic 1107	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of the structural features on the self-assembly of different poloxamines ( the conventional sequential Tetronic 304 , 901 , 904 , 908 , 1107 , 1301 , and 1307 ; a reverse-sequential counterpart Tetronic 150R1 ; and a chemically modified derivative , N-methylated Tetronic 1107 ) was thoroughly studied in 10 mM HCl by means of pi-A isotherm , surface tension , and pyrene fluorescence measurements .
	manualset3
209383	10	418156	7	NULL	NULL	0	NULL	conventional sequential Tetronic 1301	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of the structural features on the self-assembly of different poloxamines ( the conventional sequential Tetronic 304 , 901 , 904 , 908 , 1107 , 1301 , and 1307 ; a reverse-sequential counterpart Tetronic 150R1 ; and a chemically modified derivative , N-methylated Tetronic 1107 ) was thoroughly studied in 10 mM HCl by means of pi-A isotherm , surface tension , and pyrene fluorescence measurements .
	manualset3
209384	11	418156	7	NULL	NULL	0	NULL	conventional sequential Tetronic 1307	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of the structural features on the self-assembly of different poloxamines ( the conventional sequential Tetronic 304 , 901 , 904 , 908 , 1107 , 1301 , and 1307 ; a reverse-sequential counterpart Tetronic 150R1 ; and a chemically modified derivative , N-methylated Tetronic 1107 ) was thoroughly studied in 10 mM HCl by means of pi-A isotherm , surface tension , and pyrene fluorescence measurements .
	manualset3
209385	12	418156	7	NULL	NULL	0	NULL	reverse-sequential counterpart Tetronic 150R1	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of the structural features on the self-assembly of different poloxamines ( the conventional sequential Tetronic 304 , 901 , 904 , 908 , 1107 , 1301 , and 1307 ; a reverse-sequential counterpart Tetronic 150R1 ; and a chemically modified derivative , N-methylated Tetronic 1107 ) was thoroughly studied in 10 mM HCl by means of pi-A isotherm , surface tension , and pyrene fluorescence measurements .
	manualset3
209386	13	418156	7	NULL	NULL	0	NULL	chemically modified derivative , N-methylated Tetronic 1107	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of the structural features on the self-assembly of different poloxamines ( the conventional sequential Tetronic 304 , 901 , 904 , 908 , 1107 , 1301 , and 1307 ; a reverse-sequential counterpart Tetronic 150R1 ; and a chemically modified derivative , N-methylated Tetronic 1107 ) was thoroughly studied in 10 mM HCl by means of pi-A isotherm , surface tension , and pyrene fluorescence measurements .
	manualset3
209387	14	418156	7	NULL	NULL	NULL	NULL	10 mM 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The incidence of the structural features on the self-assembly of different poloxamines ( the conventional sequential Tetronic 304 , 901 , 904 , 908 , 1107 , 1301 , and 1307 ; a reverse-sequential counterpart Tetronic 150R1 ; and a chemically modified derivative , N-methylated Tetronic 1107 ) was thoroughly studied in 10 mM HCl by means of pi-A isotherm , surface tension , and pyrene fluorescence measurements .
	manualset3
209388	15	418156	7	NULL	NULL	0	NULL	pi-A isotherm	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of the structural features on the self-assembly of different poloxamines ( the conventional sequential Tetronic 304 , 901 , 904 , 908 , 1107 , 1301 , and 1307 ; a reverse-sequential counterpart Tetronic 150R1 ; and a chemically modified derivative , N-methylated Tetronic 1107 ) was thoroughly studied in 10 mM HCl by means of pi-A isotherm , surface tension , and pyrene fluorescence measurements .
	manualset3
209389	16	418156	7	NULL	NULL	0	NULL	surface tension	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of the structural features on the self-assembly of different poloxamines ( the conventional sequential Tetronic 304 , 901 , 904 , 908 , 1107 , 1301 , and 1307 ; a reverse-sequential counterpart Tetronic 150R1 ; and a chemically modified derivative , N-methylated Tetronic 1107 ) was thoroughly studied in 10 mM HCl by means of pi-A isotherm , surface tension , and pyrene fluorescence measurements .
	manualset3
209390	17	418156	7	NULL	NULL	0	NULL	pyrene fluorescence measurements	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of the structural features on the self-assembly of different poloxamines ( the conventional sequential Tetronic 304 , 901 , 904 , 908 , 1107 , 1301 , and 1307 ; a reverse-sequential counterpart Tetronic 150R1 ; and a chemically modified derivative , N-methylated Tetronic 1107 ) was thoroughly studied in 10 mM HCl by means of pi-A isotherm , surface tension , and pyrene fluorescence measurements .
	manualset3
211462	18	418156	7	NULL	NULL	0	NULL	HCl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence of the structural features on the self-assembly of different poloxamines ( the conventional sequential Tetronic 304 , 901 , 904 , 908 , 1107 , 1301 , and 1307 ; a reverse-sequential counterpart Tetronic 150R1 ; and a chemically modified derivative , N-methylated Tetronic 1107 ) was thoroughly studied in 10 mM HCl by means of pi-A isotherm , surface tension , and pyrene fluorescence measurements .
	manualset3
209391	1	418157	7	NULL	NULL	0	NULL	Subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects exhibiting absenteeism increases or persistent hypertension six months after screening were randomly assigned to worksite health education programs or no intervention .
	manualset3
209392	2	418157	7	NULL	NULL	0	NULL	absenteeism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects exhibiting absenteeism increases or persistent hypertension six months after screening were randomly assigned to worksite health education programs or no intervention .
	manualset3
209393	3	418157	7	NULL	NULL	0	NULL	persistent hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects exhibiting absenteeism increases or persistent hypertension six months after screening were randomly assigned to worksite health education programs or no intervention .
	manualset3
209394	4	418157	7	NULL	NULL	0	NULL	six months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects exhibiting absenteeism increases or persistent hypertension six months after screening were randomly assigned to worksite health education programs or no intervention .
	manualset3
209395	5	418157	7	NULL	NULL	0	NULL	screening	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects exhibiting absenteeism increases or persistent hypertension six months after screening were randomly assigned to worksite health education programs or no intervention .
	manualset3
209396	6	418157	7	NULL	NULL	0	NULL	worksite health education programs	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects exhibiting absenteeism increases or persistent hypertension six months after screening were randomly assigned to worksite health education programs or no intervention .
	manualset3
209397	7	418157	7	NULL	NULL	0	NULL	no intervention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects exhibiting absenteeism increases or persistent hypertension six months after screening were randomly assigned to worksite health education programs or no intervention .
	manualset3
209398	1	418158	7	NULL	NULL	0	NULL	 SCID-II	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The SCID-II was administered to 69 in - and outpatients on two occasions separated by 1 to 6 weeks .
	manualset3
209399	2	418158	7	NULL	NULL	0	NULL	69 in -patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The SCID-II was administered to 69 in - and outpatients on two occasions separated by 1 to 6 weeks .
	manualset3
209400	3	418158	7	NULL	NULL	0	NULL	outpatients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The SCID-II was administered to 69 in - and outpatients on two occasions separated by 1 to 6 weeks .
	manualset3
209401	4	418158	7	NULL	NULL	NULL	NULL	two occasions	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The SCID-II was administered to 69 in - and outpatients on two occasions separated by 1 to 6 weeks .
	manualset3
209402	5	418158	7	NULL	NULL	0	NULL	1 to 6 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The SCID-II was administered to 69 in - and outpatients on two occasions separated by 1 to 6 weeks .
	manualset3
209403	1	418159	7	NULL	NULL	0	NULL	11 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 11 patients ( mean interval after infarction 6 days ; 5 patients given thrombolytic therapy ) , positron emission tomography ( PET ) was performed to characterize myocardial perfusion ( with oxygen-15-labeled water ) , glucose utilization ( with fluorine-18-fluorodeoxyglucose ) and oxidative metabolism ( with carbon-11-acetate ) .
	manualset3
209404	2	418159	7	NULL	NULL	0	NULL	mean interval	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In 11 patients ( mean interval after infarction 6 days ; 5 patients given thrombolytic therapy ) , positron emission tomography ( PET ) was performed to characterize myocardial perfusion ( with oxygen-15-labeled water ) , glucose utilization ( with fluorine-18-fluorodeoxyglucose ) and oxidative metabolism ( with carbon-11-acetate ) .
	manualset3
209405	3	418159	7	NULL	NULL	0	NULL	 infarction	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In 11 patients ( mean interval after infarction 6 days ; 5 patients given thrombolytic therapy ) , positron emission tomography ( PET ) was performed to characterize myocardial perfusion ( with oxygen-15-labeled water ) , glucose utilization ( with fluorine-18-fluorodeoxyglucose ) and oxidative metabolism ( with carbon-11-acetate ) .
	manualset3
209406	4	418159	7	NULL	NULL	0	NULL	6 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In 11 patients ( mean interval after infarction 6 days ; 5 patients given thrombolytic therapy ) , positron emission tomography ( PET ) was performed to characterize myocardial perfusion ( with oxygen-15-labeled water ) , glucose utilization ( with fluorine-18-fluorodeoxyglucose ) and oxidative metabolism ( with carbon-11-acetate ) .
	manualset3
209407	5	418159	7	NULL	NULL	0	NULL	5 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 11 patients ( mean interval after infarction 6 days ; 5 patients given thrombolytic therapy ) , positron emission tomography ( PET ) was performed to characterize myocardial perfusion ( with oxygen-15-labeled water ) , glucose utilization ( with fluorine-18-fluorodeoxyglucose ) and oxidative metabolism ( with carbon-11-acetate ) .
	manualset3
209408	6	418159	7	NULL	NULL	0	NULL	 thrombolytic therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 11 patients ( mean interval after infarction 6 days ; 5 patients given thrombolytic therapy ) , positron emission tomography ( PET ) was performed to characterize myocardial perfusion ( with oxygen-15-labeled water ) , glucose utilization ( with fluorine-18-fluorodeoxyglucose ) and oxidative metabolism ( with carbon-11-acetate ) .
	manualset3
209409	7	418159	7	NULL	NULL	0	NULL	positron emission tomography ( PET )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 11 patients ( mean interval after infarction 6 days ; 5 patients given thrombolytic therapy ) , positron emission tomography ( PET ) was performed to characterize myocardial perfusion ( with oxygen-15-labeled water ) , glucose utilization ( with fluorine-18-fluorodeoxyglucose ) and oxidative metabolism ( with carbon-11-acetate ) .
	manualset3
209410	8	418159	7	NULL	NULL	0	NULL	myocardial perfusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 11 patients ( mean interval after infarction 6 days ; 5 patients given thrombolytic therapy ) , positron emission tomography ( PET ) was performed to characterize myocardial perfusion ( with oxygen-15-labeled water ) , glucose utilization ( with fluorine-18-fluorodeoxyglucose ) and oxidative metabolism ( with carbon-11-acetate ) .
	manualset3
209411	9	418159	7	NULL	NULL	0	NULL	oxygen-15-labeled water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In 11 patients ( mean interval after infarction 6 days ; 5 patients given thrombolytic therapy ) , positron emission tomography ( PET ) was performed to characterize myocardial perfusion ( with oxygen-15-labeled water ) , glucose utilization ( with fluorine-18-fluorodeoxyglucose ) and oxidative metabolism ( with carbon-11-acetate ) .
	manualset3
209412	10	418159	7	NULL	NULL	0	NULL	glucose utilization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In 11 patients ( mean interval after infarction 6 days ; 5 patients given thrombolytic therapy ) , positron emission tomography ( PET ) was performed to characterize myocardial perfusion ( with oxygen-15-labeled water ) , glucose utilization ( with fluorine-18-fluorodeoxyglucose ) and oxidative metabolism ( with carbon-11-acetate ) .
	manualset3
209413	11	418159	7	NULL	NULL	0	NULL	fluorine-18-fluorodeoxyglucose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In 11 patients ( mean interval after infarction 6 days ; 5 patients given thrombolytic therapy ) , positron emission tomography ( PET ) was performed to characterize myocardial perfusion ( with oxygen-15-labeled water ) , glucose utilization ( with fluorine-18-fluorodeoxyglucose ) and oxidative metabolism ( with carbon-11-acetate ) .
	manualset3
209414	12	418159	7	NULL	NULL	0	NULL	oxidative metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In 11 patients ( mean interval after infarction 6 days ; 5 patients given thrombolytic therapy ) , positron emission tomography ( PET ) was performed to characterize myocardial perfusion ( with oxygen-15-labeled water ) , glucose utilization ( with fluorine-18-fluorodeoxyglucose ) and oxidative metabolism ( with carbon-11-acetate ) .
	manualset3
209415	13	418159	7	NULL	NULL	0	NULL	carbon-11-acetate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In 11 patients ( mean interval after infarction 6 days ; 5 patients given thrombolytic therapy ) , positron emission tomography ( PET ) was performed to characterize myocardial perfusion ( with oxygen-15-labeled water ) , glucose utilization ( with fluorine-18-fluorodeoxyglucose ) and oxidative metabolism ( with carbon-11-acetate ) .
	manualset3
209416	1	418160	7	NULL	NULL	0	NULL	Clonazepam	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Clonazepam , a central-type benzodiazepine agonist , potentiated the GABA-induced current and the resulting hyperpolarization .
	manualset3
209417	2	418160	7	NULL	NULL	0	NULL	central-type benzodiazepine agonist	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Clonazepam , a central-type benzodiazepine agonist , potentiated the GABA-induced current and the resulting hyperpolarization .
	manualset3
209418	3	418160	7	NULL	NULL	0	NULL	GABA-induced current	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Clonazepam , a central-type benzodiazepine agonist , potentiated the GABA-induced current and the resulting hyperpolarization .
	manualset3
209419	4	418160	7	NULL	NULL	0	NULL	hyperpolarization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Clonazepam , a central-type benzodiazepine agonist , potentiated the GABA-induced current and the resulting hyperpolarization .
	manualset3
209420	1	418161	7	NULL	NULL	0	NULL	non-Hispanic whites	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to non-Hispanic whites , Hispanics had significantly lower vitamin B-12 intake and plasma concentrations ; 17 % of Hispanics and 10 % of non-Hispanic whites had concentrations & lt ; 185 pmol/L ( P & lt ; 0.05 ) .
	manualset3
209421	2	418161	7	NULL	NULL	0	NULL	Hispanics	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to non-Hispanic whites , Hispanics had significantly lower vitamin B-12 intake and plasma concentrations ; 17 % of Hispanics and 10 % of non-Hispanic whites had concentrations & lt ; 185 pmol/L ( P & lt ; 0.05 ) .
	manualset3
209422	3	418161	7	NULL	NULL	0	NULL	lower vitamin B-12 intake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to non-Hispanic whites , Hispanics had significantly lower vitamin B-12 intake and plasma concentrations ; 17 % of Hispanics and 10 % of non-Hispanic whites had concentrations & lt ; 185 pmol/L ( P & lt ; 0.05 ) .
	manualset3
209423	4	418161	7	NULL	NULL	0	NULL	plasma concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to non-Hispanic whites , Hispanics had significantly lower vitamin B-12 intake and plasma concentrations ; 17 % of Hispanics and 10 % of non-Hispanic whites had concentrations & lt ; 185 pmol/L ( P & lt ; 0.05 ) .
	manualset3
209424	5	418161	7	NULL	NULL	0	NULL	17 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to non-Hispanic whites , Hispanics had significantly lower vitamin B-12 intake and plasma concentrations ; 17 % of Hispanics and 10 % of non-Hispanic whites had concentrations & lt ; 185 pmol/L ( P & lt ; 0.05 ) .
	manualset3
209425	6	418161	7	NULL	NULL	0	NULL	Hispanics	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to non-Hispanic whites , Hispanics had significantly lower vitamin B-12 intake and plasma concentrations ; 17 % of Hispanics and 10 % of non-Hispanic whites had concentrations & lt ; 185 pmol/L ( P & lt ; 0.05 ) .
	manualset3
209426	7	418161	7	NULL	NULL	0	NULL	10 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to non-Hispanic whites , Hispanics had significantly lower vitamin B-12 intake and plasma concentrations ; 17 % of Hispanics and 10 % of non-Hispanic whites had concentrations & lt ; 185 pmol/L ( P & lt ; 0.05 ) .
	manualset3
209427	8	418161	7	NULL	NULL	0	NULL	 non-Hispanic whites	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to non-Hispanic whites , Hispanics had significantly lower vitamin B-12 intake and plasma concentrations ; 17 % of Hispanics and 10 % of non-Hispanic whites had concentrations & lt ; 185 pmol/L ( P & lt ; 0.05 ) .
	manualset3
209428	9	418161	7	NULL	NULL	0	NULL	concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to non-Hispanic whites , Hispanics had significantly lower vitamin B-12 intake and plasma concentrations ; 17 % of Hispanics and 10 % of non-Hispanic whites had concentrations & lt ; 185 pmol/L ( P & lt ; 0.05 ) .
	manualset3
209429	10	418161	7	NULL	NULL	0	NULL	& lt; 185 pmol/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to non-Hispanic whites , Hispanics had significantly lower vitamin B-12 intake and plasma concentrations ; 17 % of Hispanics and 10 % of non-Hispanic whites had concentrations & lt ; 185 pmol/L ( P & lt ; 0.05 ) .
	manualset3
209430	11	418161	7	NULL	NULL	0	NULL	P & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative to non-Hispanic whites , Hispanics had significantly lower vitamin B-12 intake and plasma concentrations ; 17 % of Hispanics and 10 % of non-Hispanic whites had concentrations & lt ; 185 pmol/L ( P & lt ; 0.05 ) .
	manualset3
209431	1	418162	7	NULL	NULL	0	NULL	Epidemiology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiology of hepatitis B virus infection in South African Chinese .
	manualset3
209432	2	418162	7	NULL	NULL	0	NULL	hepatitis B virus infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiology of hepatitis B virus infection in South African Chinese .
	manualset3
209433	3	418162	7	NULL	NULL	0	NULL	South African Chinese	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiology of hepatitis B virus infection in South African Chinese .
	manualset3
209434	1	418163	7	NULL	NULL	0	NULL	modified femoral THARIES component 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The modified femoral THARIES component was used as a preferable alternative to unipolar or bipolar hemiarthroplasty , and the results appear to be comparable in this difficult group of patients .
	manualset3
209435	2	418163	7	NULL	NULL	0	NULL	 unipolar  hemiarthroplasty	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The modified femoral THARIES component was used as a preferable alternative to unipolar or bipolar hemiarthroplasty , and the results appear to be comparable in this difficult group of patients .
	manualset3
209436	3	418163	7	NULL	NULL	0	NULL	bipolar hemiarthroplasty	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The modified femoral THARIES component was used as a preferable alternative to unipolar or bipolar hemiarthroplasty , and the results appear to be comparable in this difficult group of patients .
	manualset3
209437	4	418163	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The modified femoral THARIES component was used as a preferable alternative to unipolar or bipolar hemiarthroplasty , and the results appear to be comparable in this difficult group of patients .
	manualset3
209438	5	418163	7	NULL	NULL	0	NULL	 difficult group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The modified femoral THARIES component was used as a preferable alternative to unipolar or bipolar hemiarthroplasty , and the results appear to be comparable in this difficult group of patients .
	manualset3
209439	6	418163	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The modified femoral THARIES component was used as a preferable alternative to unipolar or bipolar hemiarthroplasty , and the results appear to be comparable in this difficult group of patients .
	manualset3
209440	1	418164	7	NULL	NULL	0	NULL	Allergic contact dermatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Allergic contact dermatitis to epoxy resin in a hemodialysis cannula .
	manualset3
209441	2	418164	7	NULL	NULL	0	NULL	epoxy resin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Allergic contact dermatitis to epoxy resin in a hemodialysis cannula .
	manualset3
209442	3	418164	7	NULL	NULL	NULL	NULL	hemodialysis cannula	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Allergic contact dermatitis to epoxy resin in a hemodialysis cannula .
	manualset3
209443	1	418165	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the activities associated with migration inhibitory factor and type II interferon , two other inhibitory activities have been found in the sera of mice infected intravenously with BCG and 3 weeks later challenged intravenously with old tuberculin .
	manualset3
209444	2	418165	7	NULL	NULL	0	NULL	 activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the activities associated with migration inhibitory factor and type II interferon , two other inhibitory activities have been found in the sera of mice infected intravenously with BCG and 3 weeks later challenged intravenously with old tuberculin .
	manualset3
209445	3	418165	7	NULL	NULL	0	NULL	 migration inhibitory factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the activities associated with migration inhibitory factor and type II interferon , two other inhibitory activities have been found in the sera of mice infected intravenously with BCG and 3 weeks later challenged intravenously with old tuberculin .
	manualset3
209446	4	418165	7	NULL	NULL	0	NULL	type II interferon	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the activities associated with migration inhibitory factor and type II interferon , two other inhibitory activities have been found in the sera of mice infected intravenously with BCG and 3 weeks later challenged intravenously with old tuberculin .
	manualset3
209447	5	418165	7	NULL	NULL	0	NULL	two other inhibitory activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the activities associated with migration inhibitory factor and type II interferon , two other inhibitory activities have been found in the sera of mice infected intravenously with BCG and 3 weeks later challenged intravenously with old tuberculin .
	manualset3
209448	6	418165	7	NULL	NULL	0	NULL	 sera	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the activities associated with migration inhibitory factor and type II interferon , two other inhibitory activities have been found in the sera of mice infected intravenously with BCG and 3 weeks later challenged intravenously with old tuberculin .
	manualset3
209449	7	418165	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the activities associated with migration inhibitory factor and type II interferon , two other inhibitory activities have been found in the sera of mice infected intravenously with BCG and 3 weeks later challenged intravenously with old tuberculin .
	manualset3
209450	8	418165	7	NULL	NULL	0	NULL	BCG 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the activities associated with migration inhibitory factor and type II interferon , two other inhibitory activities have been found in the sera of mice infected intravenously with BCG and 3 weeks later challenged intravenously with old tuberculin .
	manualset3
209451	9	418165	7	NULL	NULL	0	NULL	 3 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the activities associated with migration inhibitory factor and type II interferon , two other inhibitory activities have been found in the sera of mice infected intravenously with BCG and 3 weeks later challenged intravenously with old tuberculin .
	manualset3
209452	10	418165	7	NULL	NULL	NULL	NULL	old tuberculin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition to the activities associated with migration inhibitory factor and type II interferon , two other inhibitory activities have been found in the sera of mice infected intravenously with BCG and 3 weeks later challenged intravenously with old tuberculin .
	manualset3
209453	1	418166	7	NULL	NULL	0	NULL	 results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these results were consistent with the proposal that cAMP is a second messenger mediating relaxation of airway smooth muscle , close inspection of the data revealed a discrepancy in the relationship between cAMP accumulation and relaxation .
	manualset3
209454	2	418166	7	NULL	NULL	0	NULL	 proposal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these results were consistent with the proposal that cAMP is a second messenger mediating relaxation of airway smooth muscle , close inspection of the data revealed a discrepancy in the relationship between cAMP accumulation and relaxation .
	manualset3
209455	3	418166	7	NULL	NULL	0	NULL	cAMP 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these results were consistent with the proposal that cAMP is a second messenger mediating relaxation of airway smooth muscle , close inspection of the data revealed a discrepancy in the relationship between cAMP accumulation and relaxation .
	manualset3
209456	4	418166	7	NULL	NULL	0	NULL	second messenger	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these results were consistent with the proposal that cAMP is a second messenger mediating relaxation of airway smooth muscle , close inspection of the data revealed a discrepancy in the relationship between cAMP accumulation and relaxation .
	manualset3
209457	5	418166	7	NULL	NULL	0	NULL	relaxation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these results were consistent with the proposal that cAMP is a second messenger mediating relaxation of airway smooth muscle , close inspection of the data revealed a discrepancy in the relationship between cAMP accumulation and relaxation .
	manualset3
209458	6	418166	7	NULL	NULL	0	NULL	airway smooth muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these results were consistent with the proposal that cAMP is a second messenger mediating relaxation of airway smooth muscle , close inspection of the data revealed a discrepancy in the relationship between cAMP accumulation and relaxation .
	manualset3
209459	7	418166	7	NULL	NULL	0	NULL	close inspection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these results were consistent with the proposal that cAMP is a second messenger mediating relaxation of airway smooth muscle , close inspection of the data revealed a discrepancy in the relationship between cAMP accumulation and relaxation .
	manualset3
209460	8	418166	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these results were consistent with the proposal that cAMP is a second messenger mediating relaxation of airway smooth muscle , close inspection of the data revealed a discrepancy in the relationship between cAMP accumulation and relaxation .
	manualset3
209461	9	418166	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these results were consistent with the proposal that cAMP is a second messenger mediating relaxation of airway smooth muscle , close inspection of the data revealed a discrepancy in the relationship between cAMP accumulation and relaxation .
	manualset3
209462	10	418166	7	NULL	NULL	0	NULL	cAMP accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these results were consistent with the proposal that cAMP is a second messenger mediating relaxation of airway smooth muscle , close inspection of the data revealed a discrepancy in the relationship between cAMP accumulation and relaxation .
	manualset3
209463	11	418166	7	NULL	NULL	0	NULL	relaxation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these results were consistent with the proposal that cAMP is a second messenger mediating relaxation of airway smooth muscle , close inspection of the data revealed a discrepancy in the relationship between cAMP accumulation and relaxation .
	manualset3
209464	1	418167	7	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This study may be helpful for predicting the final cosmetic outcomes of mandibular angle ostectomy .
	manualset3
209465	2	418167	7	NULL	NULL	0	NULL	final cosmetic outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This study may be helpful for predicting the final cosmetic outcomes of mandibular angle ostectomy .
	manualset3
209466	3	418167	7	NULL	NULL	0	NULL	mandibular angle ostectomy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This study may be helpful for predicting the final cosmetic outcomes of mandibular angle ostectomy .
	manualset3
209467	1	418168	7	NULL	NULL	0	NULL	Cell culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Cell culture and animal studies have significantly contributed to our understanding of the underlying mechanisms of the association between OSAS and inflammation .
	manualset3
209468	2	418168	7	NULL	NULL	0	NULL	 animal studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Cell culture and animal studies have significantly contributed to our understanding of the underlying mechanisms of the association between OSAS and inflammation .
	manualset3
209469	3	418168	7	NULL	NULL	0	NULL	understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cell culture and animal studies have significantly contributed to our understanding of the underlying mechanisms of the association between OSAS and inflammation .
	manualset3
209470	4	418168	7	NULL	NULL	0	NULL	mechanisms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Cell culture and animal studies have significantly contributed to our understanding of the underlying mechanisms of the association between OSAS and inflammation .
	manualset3
209471	5	418168	7	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Cell culture and animal studies have significantly contributed to our understanding of the underlying mechanisms of the association between OSAS and inflammation .
	manualset3
209472	6	418168	7	NULL	NULL	0	NULL	OSAS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Cell culture and animal studies have significantly contributed to our understanding of the underlying mechanisms of the association between OSAS and inflammation .
	manualset3
209473	7	418168	7	NULL	NULL	0	NULL	inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Cell culture and animal studies have significantly contributed to our understanding of the underlying mechanisms of the association between OSAS and inflammation .
	manualset3
209474	1	418169	7	NULL	NULL	0	NULL	Converging evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Converging evidence indicates that , in controlled drug trials , individuals receiving novel antipsychotic medications have fewer adverse effects than those receiving conventional antipsychotic medications .
	manualset3
209475	2	418169	7	NULL	NULL	0	NULL	controlled drug trials	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Converging evidence indicates that , in controlled drug trials , individuals receiving novel antipsychotic medications have fewer adverse effects than those receiving conventional antipsychotic medications .
	manualset3
209476	3	418169	7	NULL	NULL	0	NULL	individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Converging evidence indicates that , in controlled drug trials , individuals receiving novel antipsychotic medications have fewer adverse effects than those receiving conventional antipsychotic medications .
	manualset3
209477	4	418169	7	NULL	NULL	0	NULL	novel antipsychotic medications	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Converging evidence indicates that , in controlled drug trials , individuals receiving novel antipsychotic medications have fewer adverse effects than those receiving conventional antipsychotic medications .
	manualset3
209478	5	418169	7	NULL	NULL	0	NULL	adverse effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Converging evidence indicates that , in controlled drug trials , individuals receiving novel antipsychotic medications have fewer adverse effects than those receiving conventional antipsychotic medications .
	manualset3
209479	6	418169	7	NULL	NULL	0	NULL	conventional antipsychotic medications	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Converging evidence indicates that , in controlled drug trials , individuals receiving novel antipsychotic medications have fewer adverse effects than those receiving conventional antipsychotic medications .
	manualset3
209480	1	418170	7	NULL	NULL	0	NULL	Theoretical considerations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical considerations and a limited body of evidence suggest a potential benefit for the use of these agents in conjunction with laser resurfacing procedures ; however , further placebo-controlled studies are needed to truly confirm these benefits .
	manualset3
209481	2	418170	7	NULL	NULL	0	NULL	evidence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical considerations and a limited body of evidence suggest a potential benefit for the use of these agents in conjunction with laser resurfacing procedures ; however , further placebo-controlled studies are needed to truly confirm these benefits .
	manualset3
209482	3	418170	7	NULL	NULL	NULL	NULL	 potential benefit	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Theoretical considerations and a limited body of evidence suggest a potential benefit for the use of these agents in conjunction with laser resurfacing procedures ; however , further placebo-controlled studies are needed to truly confirm these benefits .
	manualset3
209483	4	418170	7	NULL	NULL	0	NULL	agents 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical considerations and a limited body of evidence suggest a potential benefit for the use of these agents in conjunction with laser resurfacing procedures ; however , further placebo-controlled studies are needed to truly confirm these benefits .
	manualset3
209484	5	418170	7	NULL	NULL	0	NULL	conjunction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical considerations and a limited body of evidence suggest a potential benefit for the use of these agents in conjunction with laser resurfacing procedures ; however , further placebo-controlled studies are needed to truly confirm these benefits .
	manualset3
209485	6	418170	7	NULL	NULL	0	NULL	laser resurfacing procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical considerations and a limited body of evidence suggest a potential benefit for the use of these agents in conjunction with laser resurfacing procedures ; however , further placebo-controlled studies are needed to truly confirm these benefits .
	manualset3
209486	7	418170	7	NULL	NULL	0	NULL	placebo-controlled studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical considerations and a limited body of evidence suggest a potential benefit for the use of these agents in conjunction with laser resurfacing procedures ; however , further placebo-controlled studies are needed to truly confirm these benefits .
	manualset3
209487	8	418170	7	NULL	NULL	0	NULL	 benefits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Theoretical considerations and a limited body of evidence suggest a potential benefit for the use of these agents in conjunction with laser resurfacing procedures ; however , further placebo-controlled studies are needed to truly confirm these benefits .
	manualset3
209488	1	418171	7	NULL	NULL	0	NULL	Nitric oxide ( NO )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide ( NO ) in the spinal cord plays a role in sensory and autonomic activity .
	manualset3
209489	2	418171	7	NULL	NULL	0	NULL	spinal cord	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide ( NO ) in the spinal cord plays a role in sensory and autonomic activity .
	manualset3
209490	3	418171	7	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide ( NO ) in the spinal cord plays a role in sensory and autonomic activity .
	manualset3
209491	4	418171	7	NULL	NULL	0	NULL	 sensory activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide ( NO ) in the spinal cord plays a role in sensory and autonomic activity .
	manualset3
209492	5	418171	7	NULL	NULL	0	NULL	autonomic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitric oxide ( NO ) in the spinal cord plays a role in sensory and autonomic activity .
	manualset3
209493	1	418172	7	NULL	NULL	0	NULL	 pro-R hydrogen	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was further demonstrated that the pro-R hydrogen at C-4 of NADPH was stereospecifically utilized in this reduction .
	manualset3
209494	2	418172	7	NULL	NULL	NULL	NULL	 C-4	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was further demonstrated that the pro-R hydrogen at C-4 of NADPH was stereospecifically utilized in this reduction .
	manualset3
209495	3	418172	7	NULL	NULL	0	NULL	NADPH	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It was further demonstrated that the pro-R hydrogen at C-4 of NADPH was stereospecifically utilized in this reduction .
	manualset3
209496	4	418172	7	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was further demonstrated that the pro-R hydrogen at C-4 of NADPH was stereospecifically utilized in this reduction .
	manualset3
209497	1	418173	7	NULL	NULL	0	NULL	Chitosan	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Chitosan also serves as a three-dimensional culture substrate to facilitate cellular sphere formation among various cells but is as yet unexplored in hADSCs .
	manualset3
209498	2	418173	7	NULL	NULL	0	NULL	three-dimensional culture substrate	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Chitosan also serves as a three-dimensional culture substrate to facilitate cellular sphere formation among various cells but is as yet unexplored in hADSCs .
	manualset3
209499	3	418173	7	NULL	NULL	0	NULL	cellular sphere formation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Chitosan also serves as a three-dimensional culture substrate to facilitate cellular sphere formation among various cells but is as yet unexplored in hADSCs .
	manualset3
209500	4	418173	7	NULL	NULL	0	NULL	 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Chitosan also serves as a three-dimensional culture substrate to facilitate cellular sphere formation among various cells but is as yet unexplored in hADSCs .
	manualset3
209501	5	418173	7	NULL	NULL	0	NULL	hADSCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Chitosan also serves as a three-dimensional culture substrate to facilitate cellular sphere formation among various cells but is as yet unexplored in hADSCs .
	manualset3
209502	1	418174	7	NULL	NULL	0	NULL	Allergic inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Allergic inflammation induces a persistent mechanistic switch in thromboxane-mediated airway constriction in the mouse .
	manualset3
209503	2	418174	7	NULL	NULL	0	NULL	persistent mechanistic switch	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Allergic inflammation induces a persistent mechanistic switch in thromboxane-mediated airway constriction in the mouse .
	manualset3
209504	3	418174	7	NULL	NULL	0	NULL	thromboxane-mediated airway constriction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Allergic inflammation induces a persistent mechanistic switch in thromboxane-mediated airway constriction in the mouse .
	manualset3
209505	4	418174	7	NULL	NULL	0	NULL	mouse	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Allergic inflammation induces a persistent mechanistic switch in thromboxane-mediated airway constriction in the mouse .
	manualset3
209506	1	418175	7	NULL	NULL	0	NULL	completion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After completion of arterial phase scanning , venous structures of the liver were well visualized as seen on the venous phase .
	manualset3
209507	2	418175	7	NULL	NULL	0	NULL	arterial phase scanning	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After completion of arterial phase scanning , venous structures of the liver were well visualized as seen on the venous phase .
	manualset3
209508	3	418175	7	NULL	NULL	NULL	NULL	venous structures	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After completion of arterial phase scanning , venous structures of the liver were well visualized as seen on the venous phase .
	manualset3
209509	4	418175	7	NULL	NULL	0	NULL	 liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After completion of arterial phase scanning , venous structures of the liver were well visualized as seen on the venous phase .
	manualset3
209510	5	418175	7	NULL	NULL	0	NULL	venous phase	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After completion of arterial phase scanning , venous structures of the liver were well visualized as seen on the venous phase .
	manualset3
209511	1	418176	7	NULL	NULL	0	NULL	GATA factors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	GATA factors are zinc finger DNA binding proteins that control the development of diverse tissues by activating or repressing transcription .
	manualset3
209512	2	418176	7	NULL	NULL	0	NULL	 zinc finger DNA binding proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	GATA factors are zinc finger DNA binding proteins that control the development of diverse tissues by activating or repressing transcription .
	manualset3
209513	3	418176	7	NULL	NULL	0	NULL	development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GATA factors are zinc finger DNA binding proteins that control the development of diverse tissues by activating or repressing transcription .
	manualset3
209514	4	418176	7	NULL	NULL	0	NULL	diverse tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	GATA factors are zinc finger DNA binding proteins that control the development of diverse tissues by activating or repressing transcription .
	manualset3
209515	5	418176	7	NULL	NULL	0	NULL	activating transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GATA factors are zinc finger DNA binding proteins that control the development of diverse tissues by activating or repressing transcription .
	manualset3
209516	6	418176	7	NULL	NULL	0	NULL	repressing transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GATA factors are zinc finger DNA binding proteins that control the development of diverse tissues by activating or repressing transcription .
	manualset3
209517	1	418177	7	NULL	NULL	0	NULL	 function 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The function of the coroner 's office in relation to the physician .
	manualset3
209518	2	418177	7	NULL	NULL	0	NULL	 coroner 's office	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The function of the coroner 's office in relation to the physician .
	manualset3
209519	3	418177	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The function of the coroner 's office in relation to the physician .
	manualset3
209520	4	418177	7	NULL	NULL	0	NULL	physician	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The function of the coroner 's office in relation to the physician .
	manualset3
209521	1	418178	7	NULL	NULL	0	NULL	DL-dihydroxyphenylserine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	DL-dihydroxyphenylserine was given by mouth in a single-blind , placebo-controlled trial to two patients with orthostatic hypotension due to dopamine-beta-hydroxylase deficiency , in the hope of providing noradrenaline by endogenous decarboxylation .
	manualset3
209522	2	418178	7	NULL	NULL	0	NULL	 mouth 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	DL-dihydroxyphenylserine was given by mouth in a single-blind , placebo-controlled trial to two patients with orthostatic hypotension due to dopamine-beta-hydroxylase deficiency , in the hope of providing noradrenaline by endogenous decarboxylation .
	manualset3
209523	3	418178	7	NULL	NULL	0	NULL	single-blind , placebo-controlled trial	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	DL-dihydroxyphenylserine was given by mouth in a single-blind , placebo-controlled trial to two patients with orthostatic hypotension due to dopamine-beta-hydroxylase deficiency , in the hope of providing noradrenaline by endogenous decarboxylation .
	manualset3
209524	4	418178	7	NULL	NULL	0	NULL	two patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	DL-dihydroxyphenylserine was given by mouth in a single-blind , placebo-controlled trial to two patients with orthostatic hypotension due to dopamine-beta-hydroxylase deficiency , in the hope of providing noradrenaline by endogenous decarboxylation .
	manualset3
209525	5	418178	7	NULL	NULL	0	NULL	orthostatic hypotension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	DL-dihydroxyphenylserine was given by mouth in a single-blind , placebo-controlled trial to two patients with orthostatic hypotension due to dopamine-beta-hydroxylase deficiency , in the hope of providing noradrenaline by endogenous decarboxylation .
	manualset3
209526	6	418178	7	NULL	NULL	0	NULL	dopamine-beta-hydroxylase deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	DL-dihydroxyphenylserine was given by mouth in a single-blind , placebo-controlled trial to two patients with orthostatic hypotension due to dopamine-beta-hydroxylase deficiency , in the hope of providing noradrenaline by endogenous decarboxylation .
	manualset3
209527	7	418178	7	NULL	NULL	0	NULL	noradrenaline	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	DL-dihydroxyphenylserine was given by mouth in a single-blind , placebo-controlled trial to two patients with orthostatic hypotension due to dopamine-beta-hydroxylase deficiency , in the hope of providing noradrenaline by endogenous decarboxylation .
	manualset3
209528	8	418178	7	NULL	NULL	0	NULL	endogenous decarboxylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	DL-dihydroxyphenylserine was given by mouth in a single-blind , placebo-controlled trial to two patients with orthostatic hypotension due to dopamine-beta-hydroxylase deficiency , in the hope of providing noradrenaline by endogenous decarboxylation .
	manualset3
209529	1	418179	7	NULL	NULL	0	NULL	measurement error problem 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This can be thought of as a measurement error problem , where the distribution of errors is a mixture with a point mass at 0 .
	manualset3
209530	2	418179	7	NULL	NULL	0	NULL	distribution of errors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This can be thought of as a measurement error problem , where the distribution of errors is a mixture with a point mass at 0 .
	manualset3
209531	3	418179	7	NULL	NULL	0	NULL	point mass 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This can be thought of as a measurement error problem , where the distribution of errors is a mixture with a point mass at 0 .
	manualset3
209532	4	418179	7	NULL	NULL	0	NULL	 0	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	This can be thought of as a measurement error problem , where the distribution of errors is a mixture with a point mass at 0 .
	manualset3
209533	1	418180	7	NULL	NULL	0	NULL	Frontal assessment battery	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Frontal assessment battery and brain perfusion imaging in Alzheimer 's disease .
	manualset3
209534	2	418180	7	NULL	NULL	0	NULL	brain perfusion imaging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Frontal assessment battery and brain perfusion imaging in Alzheimer 's disease .
	manualset3
209535	3	418180	7	NULL	NULL	0	NULL	Alzheimer 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Frontal assessment battery and brain perfusion imaging in Alzheimer 's disease .
	manualset3
209536	1	418181	7	NULL	NULL	0	NULL	azido analog	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	An azido analog of quinacrine : its synthesis and utilization as a photoaffinity probe with submitochondrial particles .
	manualset3
209537	2	418181	7	NULL	NULL	0	NULL	quinacrine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	An azido analog of quinacrine : its synthesis and utilization as a photoaffinity probe with submitochondrial particles .
	manualset3
209538	3	418181	7	NULL	NULL	0	NULL	synthesis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An azido analog of quinacrine : its synthesis and utilization as a photoaffinity probe with submitochondrial particles .
	manualset3
209539	4	418181	7	NULL	NULL	0	NULL	utilization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An azido analog of quinacrine : its synthesis and utilization as a photoaffinity probe with submitochondrial particles .
	manualset3
209540	5	418181	7	NULL	NULL	0	NULL	photoaffinity probe	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	An azido analog of quinacrine : its synthesis and utilization as a photoaffinity probe with submitochondrial particles .
	manualset3
209541	6	418181	7	NULL	NULL	0	NULL	submitochondrial particles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	An azido analog of quinacrine : its synthesis and utilization as a photoaffinity probe with submitochondrial particles .
	manualset3
209542	1	418182	7	NULL	NULL	0	NULL	Therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy of refractory or recurrent childhood acute myeloid leukemia using amsacrine and etoposide with or without azacitidine : a Pediatric Oncology Group randomized phase II study .
	manualset3
209543	2	418182	7	NULL	NULL	0	NULL	refractory childhood acute myeloid leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy of refractory or recurrent childhood acute myeloid leukemia using amsacrine and etoposide with or without azacitidine : a Pediatric Oncology Group randomized phase II study .
	manualset3
209544	3	418182	7	NULL	NULL	0	NULL	 recurrent childhood acute myeloid leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy of refractory or recurrent childhood acute myeloid leukemia using amsacrine and etoposide with or without azacitidine : a Pediatric Oncology Group randomized phase II study .
	manualset3
209545	4	418182	7	NULL	NULL	0	NULL	amsacrine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy of refractory or recurrent childhood acute myeloid leukemia using amsacrine and etoposide with or without azacitidine : a Pediatric Oncology Group randomized phase II study .
	manualset3
209546	5	418182	7	NULL	NULL	0	NULL	etoposide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy of refractory or recurrent childhood acute myeloid leukemia using amsacrine and etoposide with or without azacitidine : a Pediatric Oncology Group randomized phase II study .
	manualset3
209547	6	418182	7	NULL	NULL	0	NULL	azacitidine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy of refractory or recurrent childhood acute myeloid leukemia using amsacrine and etoposide with or without azacitidine : a Pediatric Oncology Group randomized phase II study .
	manualset3
209548	7	418182	7	NULL	NULL	0	NULL	Pediatric Oncology Group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy of refractory or recurrent childhood acute myeloid leukemia using amsacrine and etoposide with or without azacitidine : a Pediatric Oncology Group randomized phase II study .
	manualset3
209549	8	418182	7	NULL	NULL	0	NULL	randomized phase II study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapy of refractory or recurrent childhood acute myeloid leukemia using amsacrine and etoposide with or without azacitidine : a Pediatric Oncology Group randomized phase II study .
	manualset3
209550	1	418183	7	NULL	NULL	0	NULL	Uterine hemangioma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Uterine hemangioma : a rare pathologic entity .
	manualset3
209551	2	418183	7	NULL	NULL	0	NULL	rare pathologic entity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Uterine hemangioma : a rare pathologic entity .
	manualset3
209552	1	418184	7	NULL	NULL	0	NULL	Allergy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Allergy as a cause of acute torticollis .
	manualset3
209553	2	418184	7	NULL	NULL	0	NULL	cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Allergy as a cause of acute torticollis .
	manualset3
209554	3	418184	7	NULL	NULL	0	NULL	acute torticollis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Allergy as a cause of acute torticollis .
	manualset3
209555	1	418185	7	NULL	NULL	0	NULL	 transfection 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , transfection of a plasmid expressing HIF-1alpha gene activates survivin gene expression and reduces the apoptotic response .
	manualset3
209556	2	418185	7	NULL	NULL	0	NULL	plasmid expressing HIF-1alpha gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	However , transfection of a plasmid expressing HIF-1alpha gene activates survivin gene expression and reduces the apoptotic response .
	manualset3
209557	3	418185	7	NULL	NULL	0	NULL	survivin gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , transfection of a plasmid expressing HIF-1alpha gene activates survivin gene expression and reduces the apoptotic response .
	manualset3
209558	4	418185	7	NULL	NULL	0	NULL	apoptotic response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , transfection of a plasmid expressing HIF-1alpha gene activates survivin gene expression and reduces the apoptotic response .
	manualset3
209559	1	418186	7	NULL	NULL	0	NULL	Pro-inflammatory cytokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Pro-inflammatory cytokines including TNF , IL-1alpha , IL-1beta and IL-1Ra cause systemic inflammatory reactions and numerous changes including altered cell signaling and migration , changes in cytokine production and fever .
	manualset3
209560	2	418186	7	NULL	NULL	0	NULL	TNF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Pro-inflammatory cytokines including TNF , IL-1alpha , IL-1beta and IL-1Ra cause systemic inflammatory reactions and numerous changes including altered cell signaling and migration , changes in cytokine production and fever .
	manualset3
209561	3	418186	7	NULL	NULL	0	NULL	IL-1alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Pro-inflammatory cytokines including TNF , IL-1alpha , IL-1beta and IL-1Ra cause systemic inflammatory reactions and numerous changes including altered cell signaling and migration , changes in cytokine production and fever .
	manualset3
209562	4	418186	7	NULL	NULL	0	NULL	IL-1beta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Pro-inflammatory cytokines including TNF , IL-1alpha , IL-1beta and IL-1Ra cause systemic inflammatory reactions and numerous changes including altered cell signaling and migration , changes in cytokine production and fever .
	manualset3
209563	5	418186	7	NULL	NULL	0	NULL	 IL-1Ra	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Pro-inflammatory cytokines including TNF , IL-1alpha , IL-1beta and IL-1Ra cause systemic inflammatory reactions and numerous changes including altered cell signaling and migration , changes in cytokine production and fever .
	manualset3
209564	6	418186	7	NULL	NULL	0	NULL	systemic inflammatory reactions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pro-inflammatory cytokines including TNF , IL-1alpha , IL-1beta and IL-1Ra cause systemic inflammatory reactions and numerous changes including altered cell signaling and migration , changes in cytokine production and fever .
	manualset3
209565	7	418186	7	NULL	NULL	0	NULL	 numerous changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pro-inflammatory cytokines including TNF , IL-1alpha , IL-1beta and IL-1Ra cause systemic inflammatory reactions and numerous changes including altered cell signaling and migration , changes in cytokine production and fever .
	manualset3
209566	8	418186	7	NULL	NULL	0	NULL	altered cell signaling	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pro-inflammatory cytokines including TNF , IL-1alpha , IL-1beta and IL-1Ra cause systemic inflammatory reactions and numerous changes including altered cell signaling and migration , changes in cytokine production and fever .
	manualset3
209567	9	418186	7	NULL	NULL	0	NULL	migration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pro-inflammatory cytokines including TNF , IL-1alpha , IL-1beta and IL-1Ra cause systemic inflammatory reactions and numerous changes including altered cell signaling and migration , changes in cytokine production and fever .
	manualset3
209568	10	418186	7	NULL	NULL	0	NULL	changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pro-inflammatory cytokines including TNF , IL-1alpha , IL-1beta and IL-1Ra cause systemic inflammatory reactions and numerous changes including altered cell signaling and migration , changes in cytokine production and fever .
	manualset3
209569	11	418186	7	NULL	NULL	0	NULL	cytokine production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pro-inflammatory cytokines including TNF , IL-1alpha , IL-1beta and IL-1Ra cause systemic inflammatory reactions and numerous changes including altered cell signaling and migration , changes in cytokine production and fever .
	manualset3
209570	12	418186	7	NULL	NULL	0	NULL	fever	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pro-inflammatory cytokines including TNF , IL-1alpha , IL-1beta and IL-1Ra cause systemic inflammatory reactions and numerous changes including altered cell signaling and migration , changes in cytokine production and fever .
	manualset3
209571	1	418187	7	NULL	NULL	0	NULL	Laser-tissue interaction modeling software 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Laser-tissue interaction modeling software can correct for this by adapting the dose applied to the skin .
	manualset3
209572	2	418187	7	NULL	NULL	0	NULL	 dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Laser-tissue interaction modeling software can correct for this by adapting the dose applied to the skin .
	manualset3
209573	3	418187	7	NULL	NULL	0	NULL	 skin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Laser-tissue interaction modeling software can correct for this by adapting the dose applied to the skin .
	manualset3
209574	1	418188	7	NULL	NULL	0	NULL	Images	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Images of contiguous 1-mm slices were acquired from apex to base with prospective and self-gated methods .
	manualset3
209575	2	418188	7	NULL	NULL	0	NULL	contiguous 1-mm slices 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Images of contiguous 1-mm slices were acquired from apex to base with prospective and self-gated methods .
	manualset3
209576	3	418188	7	NULL	NULL	0	NULL	apex	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Images of contiguous 1-mm slices were acquired from apex to base with prospective and self-gated methods .
	manualset3
209577	4	418188	7	NULL	NULL	0	NULL	base	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Images of contiguous 1-mm slices were acquired from apex to base with prospective and self-gated methods .
	manualset3
209578	5	418188	7	NULL	NULL	0	NULL	prospective methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Images of contiguous 1-mm slices were acquired from apex to base with prospective and self-gated methods .
	manualset3
209579	6	418188	7	NULL	NULL	0	NULL	self-gated methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Images of contiguous 1-mm slices were acquired from apex to base with prospective and self-gated methods .
	manualset3
209580	1	418189	7	NULL	NULL	0	NULL	Concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of PGEM in the plasma and myeloperoxidase activity ( MPO ; marker of neutrophil infiltration ) in the gut declined in 48h whereas increased iNOS activity and the macroscopic inflammatory lesions remained over the 72h follow-up period .
	manualset3
209581	2	418189	7	NULL	NULL	0	NULL	PGEM	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of PGEM in the plasma and myeloperoxidase activity ( MPO ; marker of neutrophil infiltration ) in the gut declined in 48h whereas increased iNOS activity and the macroscopic inflammatory lesions remained over the 72h follow-up period .
	manualset3
209582	3	418189	7	NULL	NULL	0	NULL	plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of PGEM in the plasma and myeloperoxidase activity ( MPO ; marker of neutrophil infiltration ) in the gut declined in 48h whereas increased iNOS activity and the macroscopic inflammatory lesions remained over the 72h follow-up period .
	manualset3
209583	4	418189	7	NULL	NULL	0	NULL	 myeloperoxidase activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of PGEM in the plasma and myeloperoxidase activity ( MPO ; marker of neutrophil infiltration ) in the gut declined in 48h whereas increased iNOS activity and the macroscopic inflammatory lesions remained over the 72h follow-up period .
	manualset3
209584	5	418189	7	NULL	NULL	0	NULL	MPO 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of PGEM in the plasma and myeloperoxidase activity ( MPO ; marker of neutrophil infiltration ) in the gut declined in 48h whereas increased iNOS activity and the macroscopic inflammatory lesions remained over the 72h follow-up period .
	manualset3
209585	6	418189	7	NULL	NULL	0	NULL	 marker of neutrophil infiltration	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of PGEM in the plasma and myeloperoxidase activity ( MPO ; marker of neutrophil infiltration ) in the gut declined in 48h whereas increased iNOS activity and the macroscopic inflammatory lesions remained over the 72h follow-up period .
	manualset3
209586	7	418189	7	NULL	NULL	0	NULL	gut	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of PGEM in the plasma and myeloperoxidase activity ( MPO ; marker of neutrophil infiltration ) in the gut declined in 48h whereas increased iNOS activity and the macroscopic inflammatory lesions remained over the 72h follow-up period .
	manualset3
209587	8	418189	7	NULL	NULL	0	NULL	 48h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of PGEM in the plasma and myeloperoxidase activity ( MPO ; marker of neutrophil infiltration ) in the gut declined in 48h whereas increased iNOS activity and the macroscopic inflammatory lesions remained over the 72h follow-up period .
	manualset3
209588	9	418189	7	NULL	NULL	0	NULL	 increased iNOS activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of PGEM in the plasma and myeloperoxidase activity ( MPO ; marker of neutrophil infiltration ) in the gut declined in 48h whereas increased iNOS activity and the macroscopic inflammatory lesions remained over the 72h follow-up period .
	manualset3
209589	10	418189	7	NULL	NULL	0	NULL	macroscopic inflammatory lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of PGEM in the plasma and myeloperoxidase activity ( MPO ; marker of neutrophil infiltration ) in the gut declined in 48h whereas increased iNOS activity and the macroscopic inflammatory lesions remained over the 72h follow-up period .
	manualset3
209590	11	418189	7	NULL	NULL	0	NULL	72h follow-up period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of PGEM in the plasma and myeloperoxidase activity ( MPO ; marker of neutrophil infiltration ) in the gut declined in 48h whereas increased iNOS activity and the macroscopic inflammatory lesions remained over the 72h follow-up period .
	manualset3
209591	1	418190	7	NULL	NULL	0	NULL	 investigation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An investigation into shivering following anaesthesia : preliminary report .
	manualset3
209592	2	418190	7	NULL	NULL	0	NULL	shivering	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An investigation into shivering following anaesthesia : preliminary report .
	manualset3
209593	3	418190	7	NULL	NULL	0	NULL	anaesthesia	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	An investigation into shivering following anaesthesia : preliminary report .
	manualset3
209594	4	418190	7	NULL	NULL	0	NULL	 preliminary report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	An investigation into shivering following anaesthesia : preliminary report .
	manualset3
209595	1	418191	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Both these patients presented an exaggerated response to TRH .
	manualset3
209596	2	418191	7	NULL	NULL	0	NULL	exaggerated response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Both these patients presented an exaggerated response to TRH .
	manualset3
209597	3	418191	7	NULL	NULL	0	NULL	TRH	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Both these patients presented an exaggerated response to TRH .
	manualset3
209598	1	418192	7	NULL	NULL	0	NULL	low pH 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	At low pH all-Ala alpha-LA is nearly as compact as wild type alpha-LA .
	manualset3
209599	2	418192	7	NULL	NULL	0	NULL	all-Ala alpha-LA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	At low pH all-Ala alpha-LA is nearly as compact as wild type alpha-LA .
	manualset3
209600	3	418192	7	NULL	NULL	0	NULL	wild type alpha-LA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	At low pH all-Ala alpha-LA is nearly as compact as wild type alpha-LA .
	manualset3
209601	1	418193	7	NULL	NULL	0	NULL	increased vascular resistance 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is now clear that an increased vascular resistance to portal blood flow is the initial factor responsible for the increase in portal pressure .
	manualset3
209602	2	418193	7	NULL	NULL	0	NULL	 portal blood flow	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is now clear that an increased vascular resistance to portal blood flow is the initial factor responsible for the increase in portal pressure .
	manualset3
209603	3	418193	7	NULL	NULL	NULL	NULL	 initial factor	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is now clear that an increased vascular resistance to portal blood flow is the initial factor responsible for the increase in portal pressure .
	manualset3
209604	4	418193	7	NULL	NULL	0	NULL	 increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It is now clear that an increased vascular resistance to portal blood flow is the initial factor responsible for the increase in portal pressure .
	manualset3
209605	5	418193	7	NULL	NULL	0	NULL	portal pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is now clear that an increased vascular resistance to portal blood flow is the initial factor responsible for the increase in portal pressure .
	manualset3
209606	1	418194	7	NULL	NULL	0	NULL	 Total hip prosthesis	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	( Total hip prosthesis of the hip joint in Norway .
	manualset3
209607	2	418194	7	NULL	NULL	0	NULL	 hip joint 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Total hip prosthesis of the hip joint in Norway .
	manualset3
209608	3	418194	7	NULL	NULL	0	NULL	Norway	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Total hip prosthesis of the hip joint in Norway .
	manualset3
209609	1	418195	7	NULL	NULL	0	NULL	Structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure of the C-terminal phosphotyrosine interaction domain of Fe65L1 complexed with the cytoplasmic tail of amyloid precursor protein reveals a novel peptide binding mode .
	manualset3
209610	2	418195	7	NULL	NULL	0	NULL	 C-terminal phosphotyrosine interaction domain 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure of the C-terminal phosphotyrosine interaction domain of Fe65L1 complexed with the cytoplasmic tail of amyloid precursor protein reveals a novel peptide binding mode .
	manualset3
209611	3	418195	7	NULL	NULL	0	NULL	Fe65L1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure of the C-terminal phosphotyrosine interaction domain of Fe65L1 complexed with the cytoplasmic tail of amyloid precursor protein reveals a novel peptide binding mode .
	manualset3
209612	4	418195	7	NULL	NULL	0	NULL	cytoplasmic tail	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure of the C-terminal phosphotyrosine interaction domain of Fe65L1 complexed with the cytoplasmic tail of amyloid precursor protein reveals a novel peptide binding mode .
	manualset3
209613	5	418195	7	NULL	NULL	0	NULL	amyloid precursor protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure of the C-terminal phosphotyrosine interaction domain of Fe65L1 complexed with the cytoplasmic tail of amyloid precursor protein reveals a novel peptide binding mode .
	manualset3
209614	6	418195	7	NULL	NULL	0	NULL	novel peptide binding mode	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure of the C-terminal phosphotyrosine interaction domain of Fe65L1 complexed with the cytoplasmic tail of amyloid precursor protein reveals a novel peptide binding mode .
	manualset3
209615	1	418196	7	NULL	NULL	0	NULL	 Italian consensus	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Italian consensus on the recommendations about the use of methotrexate for the treatment of rheumatic diseases with a focus on rheumatoid arthritis : results from the `` 3E initiative '' ) .
	manualset3
209616	2	418196	7	NULL	NULL	0	NULL	recommendations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Italian consensus on the recommendations about the use of methotrexate for the treatment of rheumatic diseases with a focus on rheumatoid arthritis : results from the `` 3E initiative '' ) .
	manualset3
209617	3	418196	7	NULL	NULL	0	NULL	methotrexate	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Italian consensus on the recommendations about the use of methotrexate for the treatment of rheumatic diseases with a focus on rheumatoid arthritis : results from the `` 3E initiative '' ) .
	manualset3
209618	4	418196	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Italian consensus on the recommendations about the use of methotrexate for the treatment of rheumatic diseases with a focus on rheumatoid arthritis : results from the `` 3E initiative '' ) .
	manualset3
209619	5	418196	7	NULL	NULL	NULL	NULL	rheumatic diseases	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Italian consensus on the recommendations about the use of methotrexate for the treatment of rheumatic diseases with a focus on rheumatoid arthritis : results from the `` 3E initiative '' ) .
	manualset3
209620	6	418196	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Italian consensus on the recommendations about the use of methotrexate for the treatment of rheumatic diseases with a focus on rheumatoid arthritis : results from the `` 3E initiative '' ) .
	manualset3
209621	7	418196	7	NULL	NULL	0	NULL	`` 3E initiative ''	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Italian consensus on the recommendations about the use of methotrexate for the treatment of rheumatic diseases with a focus on rheumatoid arthritis : results from the `` 3E initiative '' ) .
	manualset3
209622	1	418197	7	NULL	NULL	0	NULL	brain implants	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that brain implants do not need to contain dopamine to induce functional recovery in MPTP-induced parkinsonian primates .
	manualset3
209623	2	418197	7	NULL	NULL	0	NULL	dopamine	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that brain implants do not need to contain dopamine to induce functional recovery in MPTP-induced parkinsonian primates .
	manualset3
209624	3	418197	7	NULL	NULL	0	NULL	functional recovery	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that brain implants do not need to contain dopamine to induce functional recovery in MPTP-induced parkinsonian primates .
	manualset3
209625	4	418197	7	NULL	NULL	0	NULL	MPTP-induced parkinsonian primates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that brain implants do not need to contain dopamine to induce functional recovery in MPTP-induced parkinsonian primates .
	manualset3
209626	1	418198	7	NULL	NULL	0	NULL	transition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , a transition toward modern ( `` Westernized '' ) diets has led to a substantial decline of K + intake compared with traditional food habits , and a large fraction of the population might now have suboptimal K + intake .
	manualset3
209627	2	418198	7	NULL	NULL	0	NULL	modern ( `` Westernized '' ) diets	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	However , a transition toward modern ( `` Westernized '' ) diets has led to a substantial decline of K + intake compared with traditional food habits , and a large fraction of the population might now have suboptimal K + intake .
	manualset3
209628	3	418198	7	NULL	NULL	0	NULL	substantial decline	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , a transition toward modern ( `` Westernized '' ) diets has led to a substantial decline of K + intake compared with traditional food habits , and a large fraction of the population might now have suboptimal K + intake .
	manualset3
209629	4	418198	7	NULL	NULL	0	NULL	K + intake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , a transition toward modern ( `` Westernized '' ) diets has led to a substantial decline of K + intake compared with traditional food habits , and a large fraction of the population might now have suboptimal K + intake .
	manualset3
209630	5	418198	7	NULL	NULL	0	NULL	traditional food habits	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	However , a transition toward modern ( `` Westernized '' ) diets has led to a substantial decline of K + intake compared with traditional food habits , and a large fraction of the population might now have suboptimal K + intake .
	manualset3
209631	6	418198	7	NULL	NULL	0	NULL	large fraction	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , a transition toward modern ( `` Westernized '' ) diets has led to a substantial decline of K + intake compared with traditional food habits , and a large fraction of the population might now have suboptimal K + intake .
	manualset3
209632	7	418198	7	NULL	NULL	0	NULL	population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , a transition toward modern ( `` Westernized '' ) diets has led to a substantial decline of K + intake compared with traditional food habits , and a large fraction of the population might now have suboptimal K + intake .
	manualset3
209633	8	418198	7	NULL	NULL	0	NULL	suboptimal K + intake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , a transition toward modern ( `` Westernized '' ) diets has led to a substantial decline of K + intake compared with traditional food habits , and a large fraction of the population might now have suboptimal K + intake .
	manualset3
209634	1	418199	7	NULL	NULL	0	NULL	S - ( T ) 28	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	S - ( T ) 28 are poor substrates for DNA elongation catalyzed by HSV-2 DNA polymerase .
	manualset3
209635	2	418199	7	NULL	NULL	0	NULL	poor substrates	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	S - ( T ) 28 are poor substrates for DNA elongation catalyzed by HSV-2 DNA polymerase .
	manualset3
209636	3	418199	7	NULL	NULL	0	NULL	DNA elongation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	S - ( T ) 28 are poor substrates for DNA elongation catalyzed by HSV-2 DNA polymerase .
	manualset3
209637	4	418199	7	NULL	NULL	0	NULL	HSV-2 DNA polymerase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	S - ( T ) 28 are poor substrates for DNA elongation catalyzed by HSV-2 DNA polymerase .
	manualset3
209638	1	418200	7	NULL	NULL	0	NULL	degree of immunosuppression	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of immunosuppression was dependent on the dose of antigen injected iv and the time at which it was administered prior to sc sensitization .
	manualset3
209639	2	418200	7	NULL	NULL	0	NULL	dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of immunosuppression was dependent on the dose of antigen injected iv and the time at which it was administered prior to sc sensitization .
	manualset3
209640	3	418200	7	NULL	NULL	0	NULL	antigen 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of immunosuppression was dependent on the dose of antigen injected iv and the time at which it was administered prior to sc sensitization .
	manualset3
209641	4	418200	7	NULL	NULL	0	NULL	 time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of immunosuppression was dependent on the dose of antigen injected iv and the time at which it was administered prior to sc sensitization .
	manualset3
209642	5	418200	7	NULL	NULL	0	NULL	 sc sensitization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of immunosuppression was dependent on the dose of antigen injected iv and the time at which it was administered prior to sc sensitization .
	manualset3
209643	1	418201	7	NULL	NULL	NULL	NULL	diffusion coefficients 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We also calculated the diffusion coefficients of solutes such as D-glucose and ascorbic acid in the hydrogels , where we find that the diffusion coefficients of those solutes in the DN hydrogel are 60 % of that in the PEO SN and 40 % of that in the PAA SN due to its smaller effective mesh size .
	manualset3
209644	2	418201	7	NULL	NULL	0	NULL	solutes 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	We also calculated the diffusion coefficients of solutes such as D-glucose and ascorbic acid in the hydrogels , where we find that the diffusion coefficients of those solutes in the DN hydrogel are 60 % of that in the PEO SN and 40 % of that in the PAA SN due to its smaller effective mesh size .
	manualset3
209645	3	418201	7	NULL	NULL	0	NULL	D-glucose	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	We also calculated the diffusion coefficients of solutes such as D-glucose and ascorbic acid in the hydrogels , where we find that the diffusion coefficients of those solutes in the DN hydrogel are 60 % of that in the PEO SN and 40 % of that in the PAA SN due to its smaller effective mesh size .
	manualset3
209646	4	418201	7	NULL	NULL	0	NULL	ascorbic acid	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	We also calculated the diffusion coefficients of solutes such as D-glucose and ascorbic acid in the hydrogels , where we find that the diffusion coefficients of those solutes in the DN hydrogel are 60 % of that in the PEO SN and 40 % of that in the PAA SN due to its smaller effective mesh size .
	manualset3
209647	5	418201	7	NULL	NULL	0	NULL	hydrogels	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We also calculated the diffusion coefficients of solutes such as D-glucose and ascorbic acid in the hydrogels , where we find that the diffusion coefficients of those solutes in the DN hydrogel are 60 % of that in the PEO SN and 40 % of that in the PAA SN due to its smaller effective mesh size .
	manualset3
209648	6	418201	7	NULL	NULL	NULL	NULL	diffusion coefficients	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We also calculated the diffusion coefficients of solutes such as D-glucose and ascorbic acid in the hydrogels , where we find that the diffusion coefficients of those solutes in the DN hydrogel are 60 % of that in the PEO SN and 40 % of that in the PAA SN due to its smaller effective mesh size .
	manualset3
209649	7	418201	7	NULL	NULL	0	NULL	 solutes	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	We also calculated the diffusion coefficients of solutes such as D-glucose and ascorbic acid in the hydrogels , where we find that the diffusion coefficients of those solutes in the DN hydrogel are 60 % of that in the PEO SN and 40 % of that in the PAA SN due to its smaller effective mesh size .
	manualset3
209650	8	418201	7	NULL	NULL	0	NULL	DN hydrogel 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We also calculated the diffusion coefficients of solutes such as D-glucose and ascorbic acid in the hydrogels , where we find that the diffusion coefficients of those solutes in the DN hydrogel are 60 % of that in the PEO SN and 40 % of that in the PAA SN due to its smaller effective mesh size .
	manualset3
209651	9	418201	7	NULL	NULL	0	NULL	60 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We also calculated the diffusion coefficients of solutes such as D-glucose and ascorbic acid in the hydrogels , where we find that the diffusion coefficients of those solutes in the DN hydrogel are 60 % of that in the PEO SN and 40 % of that in the PAA SN due to its smaller effective mesh size .
	manualset3
209652	10	418201	7	NULL	NULL	0	NULL	PEO SN	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We also calculated the diffusion coefficients of solutes such as D-glucose and ascorbic acid in the hydrogels , where we find that the diffusion coefficients of those solutes in the DN hydrogel are 60 % of that in the PEO SN and 40 % of that in the PAA SN due to its smaller effective mesh size .
	manualset3
209653	11	418201	7	NULL	NULL	0	NULL	40 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We also calculated the diffusion coefficients of solutes such as D-glucose and ascorbic acid in the hydrogels , where we find that the diffusion coefficients of those solutes in the DN hydrogel are 60 % of that in the PEO SN and 40 % of that in the PAA SN due to its smaller effective mesh size .
	manualset3
209654	12	418201	7	NULL	NULL	0	NULL	PAA SN 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We also calculated the diffusion coefficients of solutes such as D-glucose and ascorbic acid in the hydrogels , where we find that the diffusion coefficients of those solutes in the DN hydrogel are 60 % of that in the PEO SN and 40 % of that in the PAA SN due to its smaller effective mesh size .
	manualset3
209655	13	418201	7	NULL	NULL	0	NULL	smaller effective mesh size 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We also calculated the diffusion coefficients of solutes such as D-glucose and ascorbic acid in the hydrogels , where we find that the diffusion coefficients of those solutes in the DN hydrogel are 60 % of that in the PEO SN and 40 % of that in the PAA SN due to its smaller effective mesh size .
	manualset3
209656	1	418202	7	NULL	NULL	0	NULL	Allixin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Allixin , however , was cytotoxic at higher concentrations ( ) 1 microg/ml ) .
	manualset3
209657	2	418202	7	NULL	NULL	0	NULL	 higher concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Allixin , however , was cytotoxic at higher concentrations ( ) 1 microg/ml ) .
	manualset3
209658	3	418202	7	NULL	NULL	0	NULL	1 microg/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Allixin , however , was cytotoxic at higher concentrations ( ) 1 microg/ml ) .
	manualset3
209659	1	418203	7	NULL	NULL	0	NULL	paper 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we will explore some ancient ideas about the relationship of grammar and medicine .
	manualset3
209660	2	418203	7	NULL	NULL	0	NULL	ancient ideas	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we will explore some ancient ideas about the relationship of grammar and medicine .
	manualset3
209661	3	418203	7	NULL	NULL	0	NULL	 relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we will explore some ancient ideas about the relationship of grammar and medicine .
	manualset3
209662	4	418203	7	NULL	NULL	0	NULL	grammar	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we will explore some ancient ideas about the relationship of grammar and medicine .
	manualset3
209663	5	418203	7	NULL	NULL	0	NULL	 medicine	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In this paper we will explore some ancient ideas about the relationship of grammar and medicine .
	manualset3
209664	1	418204	7	NULL	NULL	0	NULL	Prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of FOCMA antibody titer was identical ( 38 % ) in young and adult cats , indicating cats likely were exposed to FeLV as kittens because a higher prevalence of FOCMA antibody titer in older cats would otherwise be expected .
	manualset3
209665	2	418204	7	NULL	NULL	0	NULL	FOCMA antibody titer	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of FOCMA antibody titer was identical ( 38 % ) in young and adult cats , indicating cats likely were exposed to FeLV as kittens because a higher prevalence of FOCMA antibody titer in older cats would otherwise be expected .
	manualset3
209666	3	418204	7	NULL	NULL	0	NULL	38 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of FOCMA antibody titer was identical ( 38 % ) in young and adult cats , indicating cats likely were exposed to FeLV as kittens because a higher prevalence of FOCMA antibody titer in older cats would otherwise be expected .
	manualset3
209667	4	418204	7	NULL	NULL	0	NULL	 young cats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of FOCMA antibody titer was identical ( 38 % ) in young and adult cats , indicating cats likely were exposed to FeLV as kittens because a higher prevalence of FOCMA antibody titer in older cats would otherwise be expected .
	manualset3
209668	5	418204	7	NULL	NULL	0	NULL	adult cats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of FOCMA antibody titer was identical ( 38 % ) in young and adult cats , indicating cats likely were exposed to FeLV as kittens because a higher prevalence of FOCMA antibody titer in older cats would otherwise be expected .
	manualset3
209669	6	418204	7	NULL	NULL	0	NULL	cats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of FOCMA antibody titer was identical ( 38 % ) in young and adult cats , indicating cats likely were exposed to FeLV as kittens because a higher prevalence of FOCMA antibody titer in older cats would otherwise be expected .
	manualset3
209670	7	418204	7	NULL	NULL	0	NULL	FeLV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of FOCMA antibody titer was identical ( 38 % ) in young and adult cats , indicating cats likely were exposed to FeLV as kittens because a higher prevalence of FOCMA antibody titer in older cats would otherwise be expected .
	manualset3
209671	8	418204	7	NULL	NULL	0	NULL	kittens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of FOCMA antibody titer was identical ( 38 % ) in young and adult cats , indicating cats likely were exposed to FeLV as kittens because a higher prevalence of FOCMA antibody titer in older cats would otherwise be expected .
	manualset3
209672	9	418204	7	NULL	NULL	0	NULL	higher prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of FOCMA antibody titer was identical ( 38 % ) in young and adult cats , indicating cats likely were exposed to FeLV as kittens because a higher prevalence of FOCMA antibody titer in older cats would otherwise be expected .
	manualset3
209673	10	418204	7	NULL	NULL	NULL	NULL	FOCMA antibody titer	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Prevalence of FOCMA antibody titer was identical ( 38 % ) in young and adult cats , indicating cats likely were exposed to FeLV as kittens because a higher prevalence of FOCMA antibody titer in older cats would otherwise be expected .
	manualset3
209674	11	418204	7	NULL	NULL	0	NULL	older cats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of FOCMA antibody titer was identical ( 38 % ) in young and adult cats , indicating cats likely were exposed to FeLV as kittens because a higher prevalence of FOCMA antibody titer in older cats would otherwise be expected .
	manualset3
209675	1	418205	7	NULL	NULL	0	NULL	Spatial modelling	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatial modelling was applied to self-reported schistosomiasis data from over 2.5 million school students from 12 , 399 schools in all regions of mainland Tanzania .
	manualset3
209676	2	418205	7	NULL	NULL	0	NULL	self-reported schistosomiasis data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatial modelling was applied to self-reported schistosomiasis data from over 2.5 million school students from 12 , 399 schools in all regions of mainland Tanzania .
	manualset3
209677	3	418205	7	NULL	NULL	0	NULL	2.5 million school students	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatial modelling was applied to self-reported schistosomiasis data from over 2.5 million school students from 12 , 399 schools in all regions of mainland Tanzania .
	manualset3
209678	4	418205	7	NULL	NULL	0	NULL	12 , 399 schools 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatial modelling was applied to self-reported schistosomiasis data from over 2.5 million school students from 12 , 399 schools in all regions of mainland Tanzania .
	manualset3
209679	5	418205	7	NULL	NULL	0	NULL	 regions	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatial modelling was applied to self-reported schistosomiasis data from over 2.5 million school students from 12 , 399 schools in all regions of mainland Tanzania .
	manualset3
209680	6	418205	7	NULL	NULL	0	NULL	mainland Tanzania	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Spatial modelling was applied to self-reported schistosomiasis data from over 2.5 million school students from 12 , 399 schools in all regions of mainland Tanzania .
	manualset3
209681	1	418206	7	NULL	NULL	0	NULL	active compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the active compounds did not show cytotoxic activity against human cancer cell lines and no one possessed hemolytic activity , indicating that their activity is selective to pathogenic fungi and that they are not toxic at MIC concentrations .
	manualset3
209682	2	418206	7	NULL	NULL	0	NULL	cytotoxic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the active compounds did not show cytotoxic activity against human cancer cell lines and no one possessed hemolytic activity , indicating that their activity is selective to pathogenic fungi and that they are not toxic at MIC concentrations .
	manualset3
209683	3	418206	7	NULL	NULL	0	NULL	human cancer cell lines 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the active compounds did not show cytotoxic activity against human cancer cell lines and no one possessed hemolytic activity , indicating that their activity is selective to pathogenic fungi and that they are not toxic at MIC concentrations .
	manualset3
209684	4	418206	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the active compounds did not show cytotoxic activity against human cancer cell lines and no one possessed hemolytic activity , indicating that their activity is selective to pathogenic fungi and that they are not toxic at MIC concentrations .
	manualset3
209685	5	418206	7	NULL	NULL	0	NULL	hemolytic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the active compounds did not show cytotoxic activity against human cancer cell lines and no one possessed hemolytic activity , indicating that their activity is selective to pathogenic fungi and that they are not toxic at MIC concentrations .
	manualset3
209686	6	418206	7	NULL	NULL	0	NULL	activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the active compounds did not show cytotoxic activity against human cancer cell lines and no one possessed hemolytic activity , indicating that their activity is selective to pathogenic fungi and that they are not toxic at MIC concentrations .
	manualset3
209687	7	418206	7	NULL	NULL	0	NULL	pathogenic fungi 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the active compounds did not show cytotoxic activity against human cancer cell lines and no one possessed hemolytic activity , indicating that their activity is selective to pathogenic fungi and that they are not toxic at MIC concentrations .
	manualset3
209688	8	418206	7	NULL	NULL	0	NULL	 MIC concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the active compounds did not show cytotoxic activity against human cancer cell lines and no one possessed hemolytic activity , indicating that their activity is selective to pathogenic fungi and that they are not toxic at MIC concentrations .
	manualset3
209689	9	418206	7	NULL	NULL	0	NULL	toxic	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the active compounds did not show cytotoxic activity against human cancer cell lines and no one possessed hemolytic activity , indicating that their activity is selective to pathogenic fungi and that they are not toxic at MIC concentrations .
	manualset3
209690	1	418207	7	NULL	NULL	0	NULL	 alpha 1 transcripts	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas alpha 1 , beta 2 , and gamma 2 transcripts were the most abundant and ubiquitous in the rat brain -- correlating with the radioautographic distribution of GABAA receptors revealed by an ionophore ligand -- others had a more restricted expression while often being abundant .
	manualset3
209691	2	418207	7	NULL	NULL	0	NULL	beta 2 transcripts	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas alpha 1 , beta 2 , and gamma 2 transcripts were the most abundant and ubiquitous in the rat brain -- correlating with the radioautographic distribution of GABAA receptors revealed by an ionophore ligand -- others had a more restricted expression while often being abundant .
	manualset3
209692	3	418207	7	NULL	NULL	0	NULL	gamma 2 transcripts	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas alpha 1 , beta 2 , and gamma 2 transcripts were the most abundant and ubiquitous in the rat brain -- correlating with the radioautographic distribution of GABAA receptors revealed by an ionophore ligand -- others had a more restricted expression while often being abundant .
	manualset3
209693	4	418207	7	NULL	NULL	0	NULL	rat brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas alpha 1 , beta 2 , and gamma 2 transcripts were the most abundant and ubiquitous in the rat brain -- correlating with the radioautographic distribution of GABAA receptors revealed by an ionophore ligand -- others had a more restricted expression while often being abundant .
	manualset3
209694	5	418207	7	NULL	NULL	0	NULL	 radioautographic distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas alpha 1 , beta 2 , and gamma 2 transcripts were the most abundant and ubiquitous in the rat brain -- correlating with the radioautographic distribution of GABAA receptors revealed by an ionophore ligand -- others had a more restricted expression while often being abundant .
	manualset3
209695	6	418207	7	NULL	NULL	0	NULL	GABAA receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas alpha 1 , beta 2 , and gamma 2 transcripts were the most abundant and ubiquitous in the rat brain -- correlating with the radioautographic distribution of GABAA receptors revealed by an ionophore ligand -- others had a more restricted expression while often being abundant .
	manualset3
209696	7	418207	7	NULL	NULL	0	NULL	ionophore ligand 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas alpha 1 , beta 2 , and gamma 2 transcripts were the most abundant and ubiquitous in the rat brain -- correlating with the radioautographic distribution of GABAA receptors revealed by an ionophore ligand -- others had a more restricted expression while often being abundant .
	manualset3
209697	8	418207	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas alpha 1 , beta 2 , and gamma 2 transcripts were the most abundant and ubiquitous in the rat brain -- correlating with the radioautographic distribution of GABAA receptors revealed by an ionophore ligand -- others had a more restricted expression while often being abundant .
	manualset3
209698	2	418208	7	NULL	NULL	NULL	NULL	data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Combining the data on competition , pFRET and ATA effect , we suggest that the ATA sensitive anti-Leu8 and resistant anti-LAM1-3 bind to overlapping but non-identical epitopes .
	manualset3
209699	1	418208	7	NULL	NULL	0	NULL	Combining	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining the data on competition , pFRET and ATA effect , we suggest that the ATA sensitive anti-Leu8 and resistant anti-LAM1-3 bind to overlapping but non-identical epitopes .
	manualset3
209700	3	418208	7	NULL	NULL	0	NULL	competition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining the data on competition , pFRET and ATA effect , we suggest that the ATA sensitive anti-Leu8 and resistant anti-LAM1-3 bind to overlapping but non-identical epitopes .
	manualset3
209701	4	418208	7	NULL	NULL	0	NULL	pFRET effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining the data on competition , pFRET and ATA effect , we suggest that the ATA sensitive anti-Leu8 and resistant anti-LAM1-3 bind to overlapping but non-identical epitopes .
	manualset3
209702	5	418208	7	NULL	NULL	0	NULL	ATA effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining the data on competition , pFRET and ATA effect , we suggest that the ATA sensitive anti-Leu8 and resistant anti-LAM1-3 bind to overlapping but non-identical epitopes .
	manualset3
209703	6	418208	7	NULL	NULL	0	NULL	ATA sensitive anti-Leu8	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining the data on competition , pFRET and ATA effect , we suggest that the ATA sensitive anti-Leu8 and resistant anti-LAM1-3 bind to overlapping but non-identical epitopes .
	manualset3
209704	7	418208	7	NULL	NULL	0	NULL	 resistant anti-LAM1-3	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining the data on competition , pFRET and ATA effect , we suggest that the ATA sensitive anti-Leu8 and resistant anti-LAM1-3 bind to overlapping but non-identical epitopes .
	manualset3
209705	8	418208	7	NULL	NULL	0	NULL	non-identical epitopes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining the data on competition , pFRET and ATA effect , we suggest that the ATA sensitive anti-Leu8 and resistant anti-LAM1-3 bind to overlapping but non-identical epitopes .
	manualset3
209706	1	418209	7	NULL	NULL	0	NULL	extended registration framework	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An extended registration framework is presented to accurately register follow-up PET-CT study triples .
	manualset3
209707	2	418209	7	NULL	NULL	0	NULL	follow-up PET-CT study triples	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An extended registration framework is presented to accurately register follow-up PET-CT study triples .
	manualset3
209708	1	418210	7	NULL	NULL	0	NULL	Allocca et al.	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	Allocca et al. reported that AAV-5 could package an 8.9 kb vector genome .
	manualset3
209709	2	418210	7	NULL	NULL	0	NULL	AAV-5	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Allocca et al. reported that AAV-5 could package an 8.9 kb vector genome .
	manualset3
209710	3	418210	7	NULL	NULL	0	NULL	 8.9 kb vector genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Allocca et al. reported that AAV-5 could package an 8.9 kb vector genome .
	manualset3
209711	1	418211	7	NULL	NULL	0	NULL	whole body withdrawal reaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This implies that the whole body withdrawal reaction is , at least partly , a fixed act generated by a central mechanism ( a central program ) which is triggered by a sensory stimulus .
	manualset3
209712	2	418211	7	NULL	NULL	0	NULL	fixed act	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This implies that the whole body withdrawal reaction is , at least partly , a fixed act generated by a central mechanism ( a central program ) which is triggered by a sensory stimulus .
	manualset3
209713	3	418211	7	NULL	NULL	0	NULL	central mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This implies that the whole body withdrawal reaction is , at least partly , a fixed act generated by a central mechanism ( a central program ) which is triggered by a sensory stimulus .
	manualset3
209714	4	418211	7	NULL	NULL	0	NULL	central program	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This implies that the whole body withdrawal reaction is , at least partly , a fixed act generated by a central mechanism ( a central program ) which is triggered by a sensory stimulus .
	manualset3
209715	5	418211	7	NULL	NULL	0	NULL	sensory stimulus	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	This implies that the whole body withdrawal reaction is , at least partly , a fixed act generated by a central mechanism ( a central program ) which is triggered by a sensory stimulus .
	manualset3
209716	1	418212	7	NULL	NULL	0	NULL	Future developments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Future developments in the repair of these complex anomalies will rely heavily on a complete understanding of present results , which can be achieved only with attention to detail and rigorous standards .
	manualset3
209717	2	418212	7	NULL	NULL	0	NULL	repair	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Future developments in the repair of these complex anomalies will rely heavily on a complete understanding of present results , which can be achieved only with attention to detail and rigorous standards .
	manualset3
209718	3	418212	7	NULL	NULL	NULL	NULL	complex anomalies	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Future developments in the repair of these complex anomalies will rely heavily on a complete understanding of present results , which can be achieved only with attention to detail and rigorous standards .
	manualset3
209719	4	418212	7	NULL	NULL	0	NULL	complete understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Future developments in the repair of these complex anomalies will rely heavily on a complete understanding of present results , which can be achieved only with attention to detail and rigorous standards .
	manualset3
209720	5	418212	7	NULL	NULL	0	NULL	 present results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Future developments in the repair of these complex anomalies will rely heavily on a complete understanding of present results , which can be achieved only with attention to detail and rigorous standards .
	manualset3
209721	6	418212	7	NULL	NULL	0	NULL	attention	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Future developments in the repair of these complex anomalies will rely heavily on a complete understanding of present results , which can be achieved only with attention to detail and rigorous standards .
	manualset3
209722	7	418212	7	NULL	NULL	0	NULL	rigorous standards 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Future developments in the repair of these complex anomalies will rely heavily on a complete understanding of present results , which can be achieved only with attention to detail and rigorous standards .
	manualset3
209723	1	418213	7	NULL	NULL	0	NULL	SBP	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although SBP tended to decrease more with saline compared to albumin and HES , the difference was not significant .
	manualset3
209724	2	418213	7	NULL	NULL	0	NULL	saline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although SBP tended to decrease more with saline compared to albumin and HES , the difference was not significant .
	manualset3
209725	3	418213	7	NULL	NULL	0	NULL	 albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although SBP tended to decrease more with saline compared to albumin and HES , the difference was not significant .
	manualset3
209726	4	418213	7	NULL	NULL	0	NULL	HES	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although SBP tended to decrease more with saline compared to albumin and HES , the difference was not significant .
	manualset3
209727	5	418213	7	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Although SBP tended to decrease more with saline compared to albumin and HES , the difference was not significant .
	manualset3
209728	1	418214	7	NULL	NULL	0	NULL	 in vitro study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An in vitro study on human ureteric smooth muscle with the alpha1-adrenoceptor subtype blocker , tamsulosin .
	manualset3
209729	2	418214	7	NULL	NULL	0	NULL	human ureteric smooth muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An in vitro study on human ureteric smooth muscle with the alpha1-adrenoceptor subtype blocker , tamsulosin .
	manualset3
209730	3	418214	7	NULL	NULL	0	NULL	alpha1-adrenoceptor subtype blocker	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	An in vitro study on human ureteric smooth muscle with the alpha1-adrenoceptor subtype blocker , tamsulosin .
	manualset3
209731	4	418214	7	NULL	NULL	0	NULL	tamsulosin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	An in vitro study on human ureteric smooth muscle with the alpha1-adrenoceptor subtype blocker , tamsulosin .
	manualset3
209732	1	418215	7	NULL	NULL	0	NULL	Private capital	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Private capital can now be invested in the NHS .
	manualset3
209733	2	418215	7	NULL	NULL	0	NULL	 NHS	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Private capital can now be invested in the NHS .
	manualset3
209734	1	418216	7	NULL	NULL	0	NULL	Diagnostic implications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Diagnostic and prognostic implications of computed tomography of head trauma .
	manualset3
209735	2	418216	7	NULL	NULL	0	NULL	prognostic implications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Diagnostic and prognostic implications of computed tomography of head trauma .
	manualset3
209736	3	418216	7	NULL	NULL	0	NULL	computed tomography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Diagnostic and prognostic implications of computed tomography of head trauma .
	manualset3
209737	4	418216	7	NULL	NULL	0	NULL	 head trauma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Diagnostic and prognostic implications of computed tomography of head trauma .
	manualset3
209738	1	418217	7	NULL	NULL	0	NULL	bladder epithelia	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The bladder epithelia as a whole stained more strongly positive for eight lectins in the infected rats than in the control rats having a sterile silk thread in the bladder .
	manualset3
209739	2	418217	7	NULL	NULL	0	NULL	eight lectins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The bladder epithelia as a whole stained more strongly positive for eight lectins in the infected rats than in the control rats having a sterile silk thread in the bladder .
	manualset3
209740	3	418217	7	NULL	NULL	0	NULL	 infected rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The bladder epithelia as a whole stained more strongly positive for eight lectins in the infected rats than in the control rats having a sterile silk thread in the bladder .
	manualset3
209741	4	418217	7	NULL	NULL	0	NULL	control rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The bladder epithelia as a whole stained more strongly positive for eight lectins in the infected rats than in the control rats having a sterile silk thread in the bladder .
	manualset3
209742	5	418217	7	NULL	NULL	0	NULL	sterile silk thread	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The bladder epithelia as a whole stained more strongly positive for eight lectins in the infected rats than in the control rats having a sterile silk thread in the bladder .
	manualset3
209743	6	418217	7	NULL	NULL	0	NULL	bladder	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The bladder epithelia as a whole stained more strongly positive for eight lectins in the infected rats than in the control rats having a sterile silk thread in the bladder .
	manualset3
209744	1	418218	7	NULL	NULL	0	NULL	receptor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , receptor complexed with these estrogens was fully capable of binding to nuclear material , undergoing processing , and inducing PgR .
	manualset3
209745	2	418218	7	NULL	NULL	0	NULL	estrogens	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , receptor complexed with these estrogens was fully capable of binding to nuclear material , undergoing processing , and inducing PgR .
	manualset3
209746	3	418218	7	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , receptor complexed with these estrogens was fully capable of binding to nuclear material , undergoing processing , and inducing PgR .
	manualset3
209747	4	418218	7	NULL	NULL	0	NULL	 nuclear material	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	However , receptor complexed with these estrogens was fully capable of binding to nuclear material , undergoing processing , and inducing PgR .
	manualset3
209748	5	418218	7	NULL	NULL	0	NULL	processing 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , receptor complexed with these estrogens was fully capable of binding to nuclear material , undergoing processing , and inducing PgR .
	manualset3
209749	6	418218	7	NULL	NULL	0	NULL	PgR	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , receptor complexed with these estrogens was fully capable of binding to nuclear material , undergoing processing , and inducing PgR .
	manualset3
209750	1	418219	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article focuses on the current status of peptide-receptor scintigraphy in the diagnosis of lung tumors and on future developments in this field .
	manualset3
209751	2	418219	7	NULL	NULL	0	NULL	current status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article focuses on the current status of peptide-receptor scintigraphy in the diagnosis of lung tumors and on future developments in this field .
	manualset3
209752	3	418219	7	NULL	NULL	0	NULL	peptide-receptor scintigraphy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This article focuses on the current status of peptide-receptor scintigraphy in the diagnosis of lung tumors and on future developments in this field .
	manualset3
209753	4	418219	7	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article focuses on the current status of peptide-receptor scintigraphy in the diagnosis of lung tumors and on future developments in this field .
	manualset3
209754	5	418219	7	NULL	NULL	0	NULL	 lung tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This article focuses on the current status of peptide-receptor scintigraphy in the diagnosis of lung tumors and on future developments in this field .
	manualset3
209755	6	418219	7	NULL	NULL	0	NULL	future developments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article focuses on the current status of peptide-receptor scintigraphy in the diagnosis of lung tumors and on future developments in this field .
	manualset3
209756	7	418219	7	NULL	NULL	0	NULL	field	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This article focuses on the current status of peptide-receptor scintigraphy in the diagnosis of lung tumors and on future developments in this field .
	manualset3
209757	1	418220	7	NULL	NULL	0	NULL	 CZE	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that CZE can determine the level of these impurities , down to a level of 0.05 % of the main component within 15 min .
	manualset3
209758	2	418220	7	NULL	NULL	0	NULL	level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that CZE can determine the level of these impurities , down to a level of 0.05 % of the main component within 15 min .
	manualset3
209759	3	418220	7	NULL	NULL	0	NULL	 impurities	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that CZE can determine the level of these impurities , down to a level of 0.05 % of the main component within 15 min .
	manualset3
209760	4	418220	7	NULL	NULL	0	NULL	level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that CZE can determine the level of these impurities , down to a level of 0.05 % of the main component within 15 min .
	manualset3
209761	5	418220	7	NULL	NULL	0	NULL	 0.05 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that CZE can determine the level of these impurities , down to a level of 0.05 % of the main component within 15 min .
	manualset3
209762	6	418220	7	NULL	NULL	0	NULL	main component	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that CZE can determine the level of these impurities , down to a level of 0.05 % of the main component within 15 min .
	manualset3
209763	7	418220	7	NULL	NULL	0	NULL	15 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	It was shown that CZE can determine the level of these impurities , down to a level of 0.05 % of the main component within 15 min .
	manualset3
209764	1	418221	7	NULL	NULL	0	NULL	TCL1 locus	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The TCL1 locus on chromosome 14q32 .1 is frequently involved in chromosomal translocations and inversions with one of the T-cell receptor loci in human T-cell leukemias and lymphomas .
	manualset3
209765	2	418221	7	NULL	NULL	0	NULL	chromosome 14q32 .1	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The TCL1 locus on chromosome 14q32 .1 is frequently involved in chromosomal translocations and inversions with one of the T-cell receptor loci in human T-cell leukemias and lymphomas .
	manualset3
209766	3	418221	7	NULL	NULL	0	NULL	chromosomal translocations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The TCL1 locus on chromosome 14q32 .1 is frequently involved in chromosomal translocations and inversions with one of the T-cell receptor loci in human T-cell leukemias and lymphomas .
	manualset3
209767	4	418221	7	NULL	NULL	0	NULL	 inversions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The TCL1 locus on chromosome 14q32 .1 is frequently involved in chromosomal translocations and inversions with one of the T-cell receptor loci in human T-cell leukemias and lymphomas .
	manualset3
209768	5	418221	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The TCL1 locus on chromosome 14q32 .1 is frequently involved in chromosomal translocations and inversions with one of the T-cell receptor loci in human T-cell leukemias and lymphomas .
	manualset3
209769	6	418221	7	NULL	NULL	0	NULL	T-cell receptor loci	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The TCL1 locus on chromosome 14q32 .1 is frequently involved in chromosomal translocations and inversions with one of the T-cell receptor loci in human T-cell leukemias and lymphomas .
	manualset3
209770	7	418221	7	NULL	NULL	0	NULL	human T-cell leukemias	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The TCL1 locus on chromosome 14q32 .1 is frequently involved in chromosomal translocations and inversions with one of the T-cell receptor loci in human T-cell leukemias and lymphomas .
	manualset3
209771	8	418221	7	NULL	NULL	0	NULL	 lymphomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The TCL1 locus on chromosome 14q32 .1 is frequently involved in chromosomal translocations and inversions with one of the T-cell receptor loci in human T-cell leukemias and lymphomas .
	manualset3
209772	1	418222	7	NULL	NULL	0	NULL	 micro level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The micro and macro level influences affect this consciousness ; i.e. , when cultural status symbols of employment are lacking , economically disadvantaged males may establish their masculinity and enhance their status through paternity and sexual prowess .
	manualset3
209773	2	418222	7	NULL	NULL	0	NULL	macro level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The micro and macro level influences affect this consciousness ; i.e. , when cultural status symbols of employment are lacking , economically disadvantaged males may establish their masculinity and enhance their status through paternity and sexual prowess .
	manualset3
209774	3	418222	7	NULL	NULL	0	NULL	consciousness	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The micro and macro level influences affect this consciousness ; i.e. , when cultural status symbols of employment are lacking , economically disadvantaged males may establish their masculinity and enhance their status through paternity and sexual prowess .
	manualset3
209775	4	418222	7	NULL	NULL	0	NULL	cultural status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The micro and macro level influences affect this consciousness ; i.e. , when cultural status symbols of employment are lacking , economically disadvantaged males may establish their masculinity and enhance their status through paternity and sexual prowess .
	manualset3
209776	5	418222	7	NULL	NULL	0	NULL	employment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The micro and macro level influences affect this consciousness ; i.e. , when cultural status symbols of employment are lacking , economically disadvantaged males may establish their masculinity and enhance their status through paternity and sexual prowess .
	manualset3
209777	6	418222	7	NULL	NULL	0	NULL	economically disadvantaged males	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The micro and macro level influences affect this consciousness ; i.e. , when cultural status symbols of employment are lacking , economically disadvantaged males may establish their masculinity and enhance their status through paternity and sexual prowess .
	manualset3
209778	7	418222	7	NULL	NULL	0	NULL	masculinity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The micro and macro level influences affect this consciousness ; i.e. , when cultural status symbols of employment are lacking , economically disadvantaged males may establish their masculinity and enhance their status through paternity and sexual prowess .
	manualset3
209779	8	418222	7	NULL	NULL	0	NULL	status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The micro and macro level influences affect this consciousness ; i.e. , when cultural status symbols of employment are lacking , economically disadvantaged males may establish their masculinity and enhance their status through paternity and sexual prowess .
	manualset3
209780	9	418222	7	NULL	NULL	0	NULL	paternity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The micro and macro level influences affect this consciousness ; i.e. , when cultural status symbols of employment are lacking , economically disadvantaged males may establish their masculinity and enhance their status through paternity and sexual prowess .
	manualset3
209781	10	418222	7	NULL	NULL	0	NULL	sexual prowess	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The micro and macro level influences affect this consciousness ; i.e. , when cultural status symbols of employment are lacking , economically disadvantaged males may establish their masculinity and enhance their status through paternity and sexual prowess .
	manualset3
209782	1	418223	7	NULL	NULL	0	NULL	histopathology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The histopathology of active disease resembles the Arthus reaction , whereas the presence of antiepithelial cell antibodies is reminiscent of Goodpasture 's disease .
	manualset3
209783	2	418223	7	NULL	NULL	0	NULL	active disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The histopathology of active disease resembles the Arthus reaction , whereas the presence of antiepithelial cell antibodies is reminiscent of Goodpasture 's disease .
	manualset3
209784	3	418223	7	NULL	NULL	0	NULL	Arthus reaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The histopathology of active disease resembles the Arthus reaction , whereas the presence of antiepithelial cell antibodies is reminiscent of Goodpasture 's disease .
	manualset3
209785	4	418223	7	NULL	NULL	0	NULL	antiepithelial cell antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The histopathology of active disease resembles the Arthus reaction , whereas the presence of antiepithelial cell antibodies is reminiscent of Goodpasture 's disease .
	manualset3
209786	5	418223	7	NULL	NULL	0	NULL	Goodpasture 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The histopathology of active disease resembles the Arthus reaction , whereas the presence of antiepithelial cell antibodies is reminiscent of Goodpasture 's disease .
	manualset3
209787	1	418224	7	NULL	NULL	0	NULL	Anesthesia	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Anesthesia for scoliosis : dwarfism and congenitally absent odontoid process .
	manualset3
209788	2	418224	7	NULL	NULL	0	NULL	scoliosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Anesthesia for scoliosis : dwarfism and congenitally absent odontoid process .
	manualset3
209789	3	418224	7	NULL	NULL	0	NULL	dwarfism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Anesthesia for scoliosis : dwarfism and congenitally absent odontoid process .
	manualset3
209790	4	418224	7	NULL	NULL	0	NULL	congenitally absent odontoid process	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Anesthesia for scoliosis : dwarfism and congenitally absent odontoid process .
	manualset3
209791	1	418225	7	NULL	NULL	0	NULL	Electron beam computed tomography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Electron beam computed tomography : screening for coronary artery disease .
	manualset3
209792	2	418225	7	NULL	NULL	0	NULL	screening	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Electron beam computed tomography : screening for coronary artery disease .
	manualset3
209793	3	418225	7	NULL	NULL	0	NULL	coronary artery disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Electron beam computed tomography : screening for coronary artery disease .
	manualset3
209794	1	418226	7	NULL	NULL	0	NULL	Allopathic practitioners	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Allopathic practitioners often dismiss CAM because of distrust or a belief that there is no sound scientific evidence that has established its utility .
	manualset3
209795	2	418226	7	NULL	NULL	0	NULL	CAM	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Allopathic practitioners often dismiss CAM because of distrust or a belief that there is no sound scientific evidence that has established its utility .
	manualset3
209798	5	418226	7	NULL	NULL	0	NULL	scientific evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Allopathic practitioners often dismiss CAM because of distrust or a belief that there is no sound scientific evidence that has established its utility .
	manualset3
209799	6	418226	7	NULL	NULL	0	NULL	 utility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Allopathic practitioners often dismiss CAM because of distrust or a belief that there is no sound scientific evidence that has established its utility .
	manualset3
211463	7	418226	7	NULL	NULL	0	NULL	 distrust	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Allopathic practitioners often dismiss CAM because of distrust or a belief that there is no sound scientific evidence that has established its utility .
	manualset3
211464	8	418226	7	NULL	NULL	0	NULL	belief	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Allopathic practitioners often dismiss CAM because of distrust or a belief that there is no sound scientific evidence that has established its utility .
	manualset3
209800	1	418227	7	NULL	NULL	0	NULL	arrestin1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore - arrestin1 plays a central role in coupling MIF endocytosis to sustained ERK activation .
	manualset3
209801	2	418227	7	NULL	NULL	0	NULL	central role 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore - arrestin1 plays a central role in coupling MIF endocytosis to sustained ERK activation .
	manualset3
209802	3	418227	7	NULL	NULL	0	NULL	coupling MIF endocytosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore - arrestin1 plays a central role in coupling MIF endocytosis to sustained ERK activation .
	manualset3
209803	4	418227	7	NULL	NULL	0	NULL	sustained ERK activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore - arrestin1 plays a central role in coupling MIF endocytosis to sustained ERK activation .
	manualset3
209804	1	418228	7	NULL	NULL	0	NULL	MAb , M7/14	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Another MAb , M7/14 , gave profound and consistent blockade of CTL function .
	manualset3
209805	2	418228	7	NULL	NULL	0	NULL	blockade	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Another MAb , M7/14 , gave profound and consistent blockade of CTL function .
	manualset3
209806	3	418228	7	NULL	NULL	0	NULL	CTL function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Another MAb , M7/14 , gave profound and consistent blockade of CTL function .
	manualset3
209807	1	418229	7	NULL	NULL	0	NULL	Reversal potential	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversal potential for glutamate responses in hippocampal pyramidal cells .
	manualset3
209808	2	418229	7	NULL	NULL	0	NULL	glutamate responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversal potential for glutamate responses in hippocampal pyramidal cells .
	manualset3
209809	3	418229	7	NULL	NULL	0	NULL	hippocampal pyramidal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversal potential for glutamate responses in hippocampal pyramidal cells .
	manualset3
209810	1	418230	7	NULL	NULL	0	NULL	Risk of dementia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk of dementia among white and African American relatives of patients with Alzheimer disease .
	manualset3
209811	2	418230	7	NULL	NULL	0	NULL	white relatives	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk of dementia among white and African American relatives of patients with Alzheimer disease .
	manualset3
209812	3	418230	7	NULL	NULL	0	NULL	African American relatives	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk of dementia among white and African American relatives of patients with Alzheimer disease .
	manualset3
209813	4	418230	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk of dementia among white and African American relatives of patients with Alzheimer disease .
	manualset3
209814	5	418230	7	NULL	NULL	0	NULL	Alzheimer disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk of dementia among white and African American relatives of patients with Alzheimer disease .
	manualset3
209821	1	418231	7	NULL	NULL	0	NULL	Cardiac responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cardiac responses to cigarette smoking in healthy young male adults ( author 's transl ) ) .
	manualset3
209822	2	418231	7	NULL	NULL	0	NULL	cigarette smoking	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cardiac responses to cigarette smoking in healthy young male adults ( author 's transl ) ) .
	manualset3
209823	3	418231	7	NULL	NULL	0	NULL	healthy young male adults 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cardiac responses to cigarette smoking in healthy young male adults ( author 's transl ) ) .
	manualset3
209824	4	418231	7	NULL	NULL	0	NULL	author 's transl 	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cardiac responses to cigarette smoking in healthy young male adults ( author 's transl ) ) .
	manualset3
209825	1	418232	7	NULL	NULL	0	NULL	immittance components	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	None of these immittance components reaches its extremum exactly at middle-ear pressure neither at 220 nor at 660 Hz , due to the hysteresis caused by the viscoelastic behavior of the soft biological tissue of the middle-ear structures .
	manualset3
209826	2	418232	7	NULL	NULL	NULL	NULL	middle-ear pressure	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	None of these immittance components reaches its extremum exactly at middle-ear pressure neither at 220 nor at 660 Hz , due to the hysteresis caused by the viscoelastic behavior of the soft biological tissue of the middle-ear structures .
	manualset3
209827	3	418232	7	NULL	NULL	NULL	NULL	220 Hz	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	None of these immittance components reaches its extremum exactly at middle-ear pressure neither at 220 nor at 660 Hz , due to the hysteresis caused by the viscoelastic behavior of the soft biological tissue of the middle-ear structures .
	manualset3
209828	4	418232	7	NULL	NULL	0	NULL	 660 Hz	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	None of these immittance components reaches its extremum exactly at middle-ear pressure neither at 220 nor at 660 Hz , due to the hysteresis caused by the viscoelastic behavior of the soft biological tissue of the middle-ear structures .
	manualset3
209829	5	418232	7	NULL	NULL	0	NULL	hysteresis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	None of these immittance components reaches its extremum exactly at middle-ear pressure neither at 220 nor at 660 Hz , due to the hysteresis caused by the viscoelastic behavior of the soft biological tissue of the middle-ear structures .
	manualset3
209830	6	418232	7	NULL	NULL	0	NULL	viscoelastic behavior	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	None of these immittance components reaches its extremum exactly at middle-ear pressure neither at 220 nor at 660 Hz , due to the hysteresis caused by the viscoelastic behavior of the soft biological tissue of the middle-ear structures .
	manualset3
209831	7	418232	7	NULL	NULL	0	NULL	soft biological tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	None of these immittance components reaches its extremum exactly at middle-ear pressure neither at 220 nor at 660 Hz , due to the hysteresis caused by the viscoelastic behavior of the soft biological tissue of the middle-ear structures .
	manualset3
209832	8	418232	7	NULL	NULL	0	NULL	middle-ear structures	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	None of these immittance components reaches its extremum exactly at middle-ear pressure neither at 220 nor at 660 Hz , due to the hysteresis caused by the viscoelastic behavior of the soft biological tissue of the middle-ear structures .
	manualset3
209833	1	418233	7	NULL	NULL	0	NULL	Adaptation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation to tRNA acceptor stem structure by flexible adjustment in the catalytic domain of class I tRNA synthetases .
	manualset3
209834	2	418233	7	NULL	NULL	0	NULL	tRNA acceptor stem structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation to tRNA acceptor stem structure by flexible adjustment in the catalytic domain of class I tRNA synthetases .
	manualset3
209835	3	418233	7	NULL	NULL	0	NULL	flexible adjustment	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation to tRNA acceptor stem structure by flexible adjustment in the catalytic domain of class I tRNA synthetases .
	manualset3
209836	4	418233	7	NULL	NULL	0	NULL	catalytic domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation to tRNA acceptor stem structure by flexible adjustment in the catalytic domain of class I tRNA synthetases .
	manualset3
209837	5	418233	7	NULL	NULL	0	NULL	class I tRNA synthetases	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Adaptation to tRNA acceptor stem structure by flexible adjustment in the catalytic domain of class I tRNA synthetases .
	manualset3
209838	1	418234	7	NULL	NULL	0	NULL	Gastrectomy patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrectomy patients had a higher prevalence of endoscopic complications of GERD ( 58 % vs 4 % , p = 0.006 ) and of multiple prior fundoplications than those having refundoplication ( 75 % vs 24 % , p = 0.004 ) .
	manualset3
209839	2	418234	7	NULL	NULL	0	NULL	 higher prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrectomy patients had a higher prevalence of endoscopic complications of GERD ( 58 % vs 4 % , p = 0.006 ) and of multiple prior fundoplications than those having refundoplication ( 75 % vs 24 % , p = 0.004 ) .
	manualset3
209840	3	418234	7	NULL	NULL	0	NULL	 endoscopic complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrectomy patients had a higher prevalence of endoscopic complications of GERD ( 58 % vs 4 % , p = 0.006 ) and of multiple prior fundoplications than those having refundoplication ( 75 % vs 24 % , p = 0.004 ) .
	manualset3
209841	4	418234	7	NULL	NULL	0	NULL	GERD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrectomy patients had a higher prevalence of endoscopic complications of GERD ( 58 % vs 4 % , p = 0.006 ) and of multiple prior fundoplications than those having refundoplication ( 75 % vs 24 % , p = 0.004 ) .
	manualset3
209842	5	418234	7	NULL	NULL	0	NULL	58 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrectomy patients had a higher prevalence of endoscopic complications of GERD ( 58 % vs 4 % , p = 0.006 ) and of multiple prior fundoplications than those having refundoplication ( 75 % vs 24 % , p = 0.004 ) .
	manualset3
209843	6	418234	7	NULL	NULL	0	NULL	4 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrectomy patients had a higher prevalence of endoscopic complications of GERD ( 58 % vs 4 % , p = 0.006 ) and of multiple prior fundoplications than those having refundoplication ( 75 % vs 24 % , p = 0.004 ) .
	manualset3
209844	7	418234	7	NULL	NULL	0	NULL	 p = 0.006	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrectomy patients had a higher prevalence of endoscopic complications of GERD ( 58 % vs 4 % , p = 0.006 ) and of multiple prior fundoplications than those having refundoplication ( 75 % vs 24 % , p = 0.004 ) .
	manualset3
209845	8	418234	7	NULL	NULL	0	NULL	multiple prior fundoplications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrectomy patients had a higher prevalence of endoscopic complications of GERD ( 58 % vs 4 % , p = 0.006 ) and of multiple prior fundoplications than those having refundoplication ( 75 % vs 24 % , p = 0.004 ) .
	manualset3
209846	9	418234	7	NULL	NULL	0	NULL	refundoplication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrectomy patients had a higher prevalence of endoscopic complications of GERD ( 58 % vs 4 % , p = 0.006 ) and of multiple prior fundoplications than those having refundoplication ( 75 % vs 24 % , p = 0.004 ) .
	manualset3
209847	10	418234	7	NULL	NULL	0	NULL	75 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrectomy patients had a higher prevalence of endoscopic complications of GERD ( 58 % vs 4 % , p = 0.006 ) and of multiple prior fundoplications than those having refundoplication ( 75 % vs 24 % , p = 0.004 ) .
	manualset3
209848	11	418234	7	NULL	NULL	0	NULL	24 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrectomy patients had a higher prevalence of endoscopic complications of GERD ( 58 % vs 4 % , p = 0.006 ) and of multiple prior fundoplications than those having refundoplication ( 75 % vs 24 % , p = 0.004 ) .
	manualset3
209849	12	418234	7	NULL	NULL	0	NULL	p = 0.004	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Gastrectomy patients had a higher prevalence of endoscopic complications of GERD ( 58 % vs 4 % , p = 0.006 ) and of multiple prior fundoplications than those having refundoplication ( 75 % vs 24 % , p = 0.004 ) .
	manualset3
209850	1	418235	7	NULL	NULL	0	NULL	microslab gel electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	By combining microslab gel electrophoresis , 30 min electrophoretic transfer , and glutaraldehyde fixation of nitrocellulose paper , an immunoblot analysis can be done in an 8-hr day .
	manualset3
209851	2	418235	7	NULL	NULL	0	NULL	30 min 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	By combining microslab gel electrophoresis , 30 min electrophoretic transfer , and glutaraldehyde fixation of nitrocellulose paper , an immunoblot analysis can be done in an 8-hr day .
	manualset3
209852	3	418235	7	NULL	NULL	0	NULL	 electrophoretic transfer	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	By combining microslab gel electrophoresis , 30 min electrophoretic transfer , and glutaraldehyde fixation of nitrocellulose paper , an immunoblot analysis can be done in an 8-hr day .
	manualset3
209853	4	418235	7	NULL	NULL	0	NULL	glutaraldehyde fixation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	By combining microslab gel electrophoresis , 30 min electrophoretic transfer , and glutaraldehyde fixation of nitrocellulose paper , an immunoblot analysis can be done in an 8-hr day .
	manualset3
209854	5	418235	7	NULL	NULL	0	NULL	nitrocellulose paper	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	By combining microslab gel electrophoresis , 30 min electrophoretic transfer , and glutaraldehyde fixation of nitrocellulose paper , an immunoblot analysis can be done in an 8-hr day .
	manualset3
209855	6	418235	7	NULL	NULL	0	NULL	 immunoblot analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	By combining microslab gel electrophoresis , 30 min electrophoretic transfer , and glutaraldehyde fixation of nitrocellulose paper , an immunoblot analysis can be done in an 8-hr day .
	manualset3
209856	7	418235	7	NULL	NULL	0	NULL	8-hr day	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	By combining microslab gel electrophoresis , 30 min electrophoretic transfer , and glutaraldehyde fixation of nitrocellulose paper , an immunoblot analysis can be done in an 8-hr day .
	manualset3
209857	1	418236	7	NULL	NULL	NULL	NULL	Allostery	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Allostery and the dynamic oligomerization of porphobilinogen synthase .
	manualset3
209858	2	418236	7	NULL	NULL	0	NULL	dynamic oligomerization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Allostery and the dynamic oligomerization of porphobilinogen synthase .
	manualset3
209859	3	418236	7	NULL	NULL	0	NULL	porphobilinogen synthase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Allostery and the dynamic oligomerization of porphobilinogen synthase .
	manualset3
209860	1	418237	7	NULL	NULL	0	NULL	 44 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In 44 ( or 21 % ) exists an extreme left axis deviation before or after operation on congenital heart malformations .
	manualset3
209861	2	418237	7	NULL	NULL	0	NULL	21 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 44 ( or 21 % ) exists an extreme left axis deviation before or after operation on congenital heart malformations .
	manualset3
209862	3	418237	7	NULL	NULL	0	NULL	extreme left axis deviation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 44 ( or 21 % ) exists an extreme left axis deviation before or after operation on congenital heart malformations .
	manualset3
209863	4	418237	7	NULL	NULL	0	NULL	operation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 44 ( or 21 % ) exists an extreme left axis deviation before or after operation on congenital heart malformations .
	manualset3
209864	5	418237	7	NULL	NULL	0	NULL	congenital heart malformations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 44 ( or 21 % ) exists an extreme left axis deviation before or after operation on congenital heart malformations .
	manualset3
209865	1	418238	7	NULL	NULL	0	NULL	G. intestinalis ) infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	G. intestinalis ) infection in young adults leads to acute/chronic diarrhea in some individuals and is asymptomatic in others .
	manualset3
209866	2	418238	7	NULL	NULL	0	NULL	young adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	G. intestinalis ) infection in young adults leads to acute/chronic diarrhea in some individuals and is asymptomatic in others .
	manualset3
209867	3	418238	7	NULL	NULL	0	NULL	acute/chronic diarrhea	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	G. intestinalis ) infection in young adults leads to acute/chronic diarrhea in some individuals and is asymptomatic in others .
	manualset3
209868	4	418238	7	NULL	NULL	0	NULL	 individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	G. intestinalis ) infection in young adults leads to acute/chronic diarrhea in some individuals and is asymptomatic in others .
	manualset3
209869	1	418239	7	NULL	NULL	0	NULL	 fragment Agp1-M20	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The fragment Agp1-M20 , which is derived from Agp1-M15 by truncation of the C-terminal `` PHY domain '' ( 191 amino acids ) , can also form dimers , but dimerization is independent of irradiation conditions .
	manualset3
209870	2	418239	7	NULL	NULL	NULL	NULL	Agp1-M15	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The fragment Agp1-M20 , which is derived from Agp1-M15 by truncation of the C-terminal `` PHY domain '' ( 191 amino acids ) , can also form dimers , but dimerization is independent of irradiation conditions .
	manualset3
209871	3	418239	7	NULL	NULL	0	NULL	 truncation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The fragment Agp1-M20 , which is derived from Agp1-M15 by truncation of the C-terminal `` PHY domain '' ( 191 amino acids ) , can also form dimers , but dimerization is independent of irradiation conditions .
	manualset3
209872	4	418239	7	NULL	NULL	0	NULL	C-terminal `` PHY domain '' 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The fragment Agp1-M20 , which is derived from Agp1-M15 by truncation of the C-terminal `` PHY domain '' ( 191 amino acids ) , can also form dimers , but dimerization is independent of irradiation conditions .
	manualset3
209873	5	418239	7	NULL	NULL	0	NULL	191 amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The fragment Agp1-M20 , which is derived from Agp1-M15 by truncation of the C-terminal `` PHY domain '' ( 191 amino acids ) , can also form dimers , but dimerization is independent of irradiation conditions .
	manualset3
209874	6	418239	7	NULL	NULL	0	NULL	dimers	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The fragment Agp1-M20 , which is derived from Agp1-M15 by truncation of the C-terminal `` PHY domain '' ( 191 amino acids ) , can also form dimers , but dimerization is independent of irradiation conditions .
	manualset3
209875	7	418239	7	NULL	NULL	0	NULL	dimerization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The fragment Agp1-M20 , which is derived from Agp1-M15 by truncation of the C-terminal `` PHY domain '' ( 191 amino acids ) , can also form dimers , but dimerization is independent of irradiation conditions .
	manualset3
209876	8	418239	7	NULL	NULL	0	NULL	irradiation conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The fragment Agp1-M20 , which is derived from Agp1-M15 by truncation of the C-terminal `` PHY domain '' ( 191 amino acids ) , can also form dimers , but dimerization is independent of irradiation conditions .
	manualset3
209877	1	418240	7	NULL	NULL	0	NULL	second protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The second protein had no immunological cross-reactivity with the known proteins or organ extracts which were tested .
	manualset3
209878	2	418240	7	NULL	NULL	0	NULL	immunological cross-reactivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The second protein had no immunological cross-reactivity with the known proteins or organ extracts which were tested .
	manualset3
209879	3	418240	7	NULL	NULL	0	NULL	proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The second protein had no immunological cross-reactivity with the known proteins or organ extracts which were tested .
	manualset3
209880	4	418240	7	NULL	NULL	NULL	NULL	organ extracts	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The second protein had no immunological cross-reactivity with the known proteins or organ extracts which were tested .
	manualset3
209881	1	418241	7	NULL	NULL	0	NULL	meconium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence or absence of meconium was noted in the prolonged-pregnancy group and correlated with the above morphological features .
	manualset3
209882	2	418241	7	NULL	NULL	0	NULL	prolonged-pregnancy group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence or absence of meconium was noted in the prolonged-pregnancy group and correlated with the above morphological features .
	manualset3
209883	3	418241	7	NULL	NULL	0	NULL	morphological features	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence or absence of meconium was noted in the prolonged-pregnancy group and correlated with the above morphological features .
	manualset3
209884	1	418242	7	NULL	NULL	0	NULL	control group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The control group was selected from daytime workers .
	manualset3
209885	2	418242	7	NULL	NULL	0	NULL	daytime workers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The control group was selected from daytime workers .
	manualset3
209886	1	418243	7	NULL	NULL	NULL	NULL	Anatomical aspects	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Anatomical and functional aspects of the HMC predispose it to injury , including the fact that the muscles cross two joints and undergo eccentric contraction during the gait cycle .
	manualset3
209887	2	418243	7	NULL	NULL	0	NULL	functional aspects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomical and functional aspects of the HMC predispose it to injury , including the fact that the muscles cross two joints and undergo eccentric contraction during the gait cycle .
	manualset3
209888	3	418243	7	NULL	NULL	0	NULL	HMC	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomical and functional aspects of the HMC predispose it to injury , including the fact that the muscles cross two joints and undergo eccentric contraction during the gait cycle .
	manualset3
209889	4	418243	7	NULL	NULL	0	NULL	injury 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomical and functional aspects of the HMC predispose it to injury , including the fact that the muscles cross two joints and undergo eccentric contraction during the gait cycle .
	manualset3
209890	5	418243	7	NULL	NULL	NULL	NULL	muscles 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Anatomical and functional aspects of the HMC predispose it to injury , including the fact that the muscles cross two joints and undergo eccentric contraction during the gait cycle .
	manualset3
209891	6	418243	7	NULL	NULL	0	NULL	eccentric contraction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomical and functional aspects of the HMC predispose it to injury , including the fact that the muscles cross two joints and undergo eccentric contraction during the gait cycle .
	manualset3
209892	7	418243	7	NULL	NULL	0	NULL	gait cycle	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomical and functional aspects of the HMC predispose it to injury , including the fact that the muscles cross two joints and undergo eccentric contraction during the gait cycle .
	manualset3
210682	8	418243	7	NULL	NULL	0	NULL	two joints	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomical and functional aspects of the HMC predispose it to injury , including the fact that the muscles cross two joints and undergo eccentric contraction during the gait cycle .
	manualset3
209893	1	418244	7	NULL	NULL	0	NULL	Indicators	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Indicators of lean body mass catabolism : emphasis on the creatinine excretion rate .
	manualset3
209894	2	418244	7	NULL	NULL	0	NULL	 lean body mass catabolism 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Indicators of lean body mass catabolism : emphasis on the creatinine excretion rate .
	manualset3
209895	3	418244	7	NULL	NULL	0	NULL	emphasis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Indicators of lean body mass catabolism : emphasis on the creatinine excretion rate .
	manualset3
209896	4	418244	7	NULL	NULL	0	NULL	creatinine excretion rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Indicators of lean body mass catabolism : emphasis on the creatinine excretion rate .
	manualset3
209897	1	418245	7	NULL	NULL	0	NULL	 chronic cannabis abuse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is plausible that chronic cannabis abuse will then interfere with educational and vocational training .
	manualset3
209898	2	418245	7	NULL	NULL	0	NULL	educational training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is plausible that chronic cannabis abuse will then interfere with educational and vocational training .
	manualset3
209899	3	418245	7	NULL	NULL	0	NULL	vocational training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is plausible that chronic cannabis abuse will then interfere with educational and vocational training .
	manualset3
209900	1	418246	7	NULL	NULL	0	NULL	context-dependent mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Allowing context-dependent mutation provides a better fit to coding sequence data than simpler ( context-independent or CpG `` hotspot '' ) models and significantly affects selection parameter estimates .
	manualset3
209901	2	418246	7	NULL	NULL	0	NULL	coding sequence data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Allowing context-dependent mutation provides a better fit to coding sequence data than simpler ( context-independent or CpG `` hotspot '' ) models and significantly affects selection parameter estimates .
	manualset3
209902	3	418246	7	NULL	NULL	0	NULL	simpler models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Allowing context-dependent mutation provides a better fit to coding sequence data than simpler ( context-independent or CpG `` hotspot '' ) models and significantly affects selection parameter estimates .
	manualset3
209903	4	418246	7	NULL	NULL	0	NULL	context-independent	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Allowing context-dependent mutation provides a better fit to coding sequence data than simpler ( context-independent or CpG `` hotspot '' ) models and significantly affects selection parameter estimates .
	manualset3
209904	5	418246	7	NULL	NULL	0	NULL	CpG `` hotspot ''	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Allowing context-dependent mutation provides a better fit to coding sequence data than simpler ( context-independent or CpG `` hotspot '' ) models and significantly affects selection parameter estimates .
	manualset3
209905	6	418246	7	NULL	NULL	0	NULL	selection parameter estimates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Allowing context-dependent mutation provides a better fit to coding sequence data than simpler ( context-independent or CpG `` hotspot '' ) models and significantly affects selection parameter estimates .
	manualset3
209906	1	418247	7	NULL	NULL	0	NULL	 serotonin agonist	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The serotonin agonist , sumatriptan , is a new , highly promising alternative treatment for migraine that has a vasoconstricting effect on the blood vessels dilated during an attack .
	manualset3
209907	2	418247	7	NULL	NULL	0	NULL	 sumatriptan	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The serotonin agonist , sumatriptan , is a new , highly promising alternative treatment for migraine that has a vasoconstricting effect on the blood vessels dilated during an attack .
	manualset3
209908	3	418247	7	NULL	NULL	0	NULL	alternative treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The serotonin agonist , sumatriptan , is a new , highly promising alternative treatment for migraine that has a vasoconstricting effect on the blood vessels dilated during an attack .
	manualset3
209909	4	418247	7	NULL	NULL	0	NULL	 migraine	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The serotonin agonist , sumatriptan , is a new , highly promising alternative treatment for migraine that has a vasoconstricting effect on the blood vessels dilated during an attack .
	manualset3
209910	5	418247	7	NULL	NULL	0	NULL	vasoconstricting effect 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The serotonin agonist , sumatriptan , is a new , highly promising alternative treatment for migraine that has a vasoconstricting effect on the blood vessels dilated during an attack .
	manualset3
209911	6	418247	7	NULL	NULL	0	NULL	blood vessels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The serotonin agonist , sumatriptan , is a new , highly promising alternative treatment for migraine that has a vasoconstricting effect on the blood vessels dilated during an attack .
	manualset3
209912	7	418247	7	NULL	NULL	0	NULL	attack	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The serotonin agonist , sumatriptan , is a new , highly promising alternative treatment for migraine that has a vasoconstricting effect on the blood vessels dilated during an attack .
	manualset3
209913	1	418248	7	NULL	NULL	0	NULL	 review 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of human milk banking and public health policy in Australia .
	manualset3
209914	2	418248	7	NULL	NULL	0	NULL	human milk banking	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of human milk banking and public health policy in Australia .
	manualset3
209915	3	418248	7	NULL	NULL	0	NULL	public health policy 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of human milk banking and public health policy in Australia .
	manualset3
209916	4	418248	7	NULL	NULL	0	NULL	Australia	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A review of human milk banking and public health policy in Australia .
	manualset3
209917	1	418249	7	NULL	NULL	0	NULL	Epidemiology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiology , clinical signs , pathology , diagnosis , prevention and control are described .
	manualset3
209918	2	418249	7	NULL	NULL	0	NULL	clinical signs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiology , clinical signs , pathology , diagnosis , prevention and control are described .
	manualset3
209919	3	418249	7	NULL	NULL	0	NULL	pathology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiology , clinical signs , pathology , diagnosis , prevention and control are described .
	manualset3
209920	4	418249	7	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiology , clinical signs , pathology , diagnosis , prevention and control are described .
	manualset3
209921	5	418249	7	NULL	NULL	0	NULL	 prevention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiology , clinical signs , pathology , diagnosis , prevention and control are described .
	manualset3
209922	6	418249	7	NULL	NULL	0	NULL	control 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiology , clinical signs , pathology , diagnosis , prevention and control are described .
	manualset3
209923	1	418250	7	NULL	NULL	0	NULL	Macrophage KLF4 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Macrophage KLF4 expression was robustly induced in M2 macrophages and strongly reduced in M1 macrophages , observations that were recapitulated in human inflammatory paradigms in vivo .
	manualset3
209924	2	418250	7	NULL	NULL	0	NULL	M2 macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Macrophage KLF4 expression was robustly induced in M2 macrophages and strongly reduced in M1 macrophages , observations that were recapitulated in human inflammatory paradigms in vivo .
	manualset3
209925	3	418250	7	NULL	NULL	0	NULL	M1 macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Macrophage KLF4 expression was robustly induced in M2 macrophages and strongly reduced in M1 macrophages , observations that were recapitulated in human inflammatory paradigms in vivo .
	manualset3
209926	4	418250	7	NULL	NULL	0	NULL	observations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Macrophage KLF4 expression was robustly induced in M2 macrophages and strongly reduced in M1 macrophages , observations that were recapitulated in human inflammatory paradigms in vivo .
	manualset3
209927	5	418250	7	NULL	NULL	0	NULL	human inflammatory paradigms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Macrophage KLF4 expression was robustly induced in M2 macrophages and strongly reduced in M1 macrophages , observations that were recapitulated in human inflammatory paradigms in vivo .
	manualset3
209928	1	418251	7	NULL	NULL	0	NULL	revenue	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This revenue could be used to reduce the costs of improved land management by three quarters or double the number of biodiversity targets achieved and meet carbon storage targets for the same cost .
	manualset3
209929	2	418251	7	NULL	NULL	0	NULL	costs	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This revenue could be used to reduce the costs of improved land management by three quarters or double the number of biodiversity targets achieved and meet carbon storage targets for the same cost .
	manualset3
209930	3	418251	7	NULL	NULL	0	NULL	land management 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This revenue could be used to reduce the costs of improved land management by three quarters or double the number of biodiversity targets achieved and meet carbon storage targets for the same cost .
	manualset3
209931	4	418251	7	NULL	NULL	0	NULL	three quarters	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	This revenue could be used to reduce the costs of improved land management by three quarters or double the number of biodiversity targets achieved and meet carbon storage targets for the same cost .
	manualset3
209932	5	418251	7	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This revenue could be used to reduce the costs of improved land management by three quarters or double the number of biodiversity targets achieved and meet carbon storage targets for the same cost .
	manualset3
209933	6	418251	7	NULL	NULL	0	NULL	 biodiversity targets	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	This revenue could be used to reduce the costs of improved land management by three quarters or double the number of biodiversity targets achieved and meet carbon storage targets for the same cost .
	manualset3
209934	7	418251	7	NULL	NULL	0	NULL	carbon storage targets	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This revenue could be used to reduce the costs of improved land management by three quarters or double the number of biodiversity targets achieved and meet carbon storage targets for the same cost .
	manualset3
209935	8	418251	7	NULL	NULL	0	NULL	 cost 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This revenue could be used to reduce the costs of improved land management by three quarters or double the number of biodiversity targets achieved and meet carbon storage targets for the same cost .
	manualset3
209936	1	418252	7	NULL	NULL	0	NULL	Cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells expressing M2 from multicopy plasmids have reduced growth rates , suggesting that high levels of M2 are toxic to growth .
	manualset3
209937	2	418252	7	NULL	NULL	0	NULL	M2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells expressing M2 from multicopy plasmids have reduced growth rates , suggesting that high levels of M2 are toxic to growth .
	manualset3
209938	3	418252	7	NULL	NULL	0	NULL	multicopy plasmids	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells expressing M2 from multicopy plasmids have reduced growth rates , suggesting that high levels of M2 are toxic to growth .
	manualset3
209939	4	418252	7	NULL	NULL	0	NULL	growth rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells expressing M2 from multicopy plasmids have reduced growth rates , suggesting that high levels of M2 are toxic to growth .
	manualset3
209940	5	418252	7	NULL	NULL	0	NULL	high levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells expressing M2 from multicopy plasmids have reduced growth rates , suggesting that high levels of M2 are toxic to growth .
	manualset3
209941	6	418252	7	NULL	NULL	0	NULL	M2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells expressing M2 from multicopy plasmids have reduced growth rates , suggesting that high levels of M2 are toxic to growth .
	manualset3
209942	7	418252	7	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells expressing M2 from multicopy plasmids have reduced growth rates , suggesting that high levels of M2 are toxic to growth .
	manualset3
209943	1	418253	7	NULL	NULL	0	NULL	 results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that 14S , 21R-diHDHA activates the p38 MAPK pathway in wounds , db/db MSCs , and DMVECs .
	manualset3
209944	2	418253	7	NULL	NULL	0	NULL	14S , 21R-diHDHA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that 14S , 21R-diHDHA activates the p38 MAPK pathway in wounds , db/db MSCs , and DMVECs .
	manualset3
209945	3	418253	7	NULL	NULL	0	NULL	p38 MAPK pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that 14S , 21R-diHDHA activates the p38 MAPK pathway in wounds , db/db MSCs , and DMVECs .
	manualset3
209946	4	418253	7	NULL	NULL	0	NULL	wounds 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that 14S , 21R-diHDHA activates the p38 MAPK pathway in wounds , db/db MSCs , and DMVECs .
	manualset3
209947	5	418253	7	NULL	NULL	0	NULL	db/db MSCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that 14S , 21R-diHDHA activates the p38 MAPK pathway in wounds , db/db MSCs , and DMVECs .
	manualset3
209948	6	418253	7	NULL	NULL	0	NULL	DMVECs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that 14S , 21R-diHDHA activates the p38 MAPK pathway in wounds , db/db MSCs , and DMVECs .
	manualset3
209949	1	418254	7	NULL	NULL	0	NULL	Macroscopic spatial analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Macroscopic spatial analysis of pedestrian and bicycle crashes .
	manualset3
209950	2	418254	7	NULL	NULL	0	NULL	pedestrian	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Macroscopic spatial analysis of pedestrian and bicycle crashes .
	manualset3
209951	3	418254	7	NULL	NULL	0	NULL	bicycle crashes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Macroscopic spatial analysis of pedestrian and bicycle crashes .
	manualset3
209952	1	418255	7	NULL	NULL	0	NULL	Retinal stem/progenitor properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinal stem/progenitor properties were also isolated from the ciliary body ( CB ) of the eye where , as in the CNS , such stem/progenitors also form spheres and have been considered to expand only via expansion by their proliferation even from the single-cell level ( called spheres of pigment cells from the ciliary margin : PCM-spheres ) .
	manualset3
209953	2	418255	7	NULL	NULL	0	NULL	 ciliary body ( CB ) 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinal stem/progenitor properties were also isolated from the ciliary body ( CB ) of the eye where , as in the CNS , such stem/progenitors also form spheres and have been considered to expand only via expansion by their proliferation even from the single-cell level ( called spheres of pigment cells from the ciliary margin : PCM-spheres ) .
	manualset3
209954	3	418255	7	NULL	NULL	0	NULL	eye	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinal stem/progenitor properties were also isolated from the ciliary body ( CB ) of the eye where , as in the CNS , such stem/progenitors also form spheres and have been considered to expand only via expansion by their proliferation even from the single-cell level ( called spheres of pigment cells from the ciliary margin : PCM-spheres ) .
	manualset3
209955	4	418255	7	NULL	NULL	0	NULL	 CNS	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinal stem/progenitor properties were also isolated from the ciliary body ( CB ) of the eye where , as in the CNS , such stem/progenitors also form spheres and have been considered to expand only via expansion by their proliferation even from the single-cell level ( called spheres of pigment cells from the ciliary margin : PCM-spheres ) .
	manualset3
209956	5	418255	7	NULL	NULL	0	NULL	 stem/progenitors	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinal stem/progenitor properties were also isolated from the ciliary body ( CB ) of the eye where , as in the CNS , such stem/progenitors also form spheres and have been considered to expand only via expansion by their proliferation even from the single-cell level ( called spheres of pigment cells from the ciliary margin : PCM-spheres ) .
	manualset3
209957	6	418255	7	NULL	NULL	0	NULL	spheres	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinal stem/progenitor properties were also isolated from the ciliary body ( CB ) of the eye where , as in the CNS , such stem/progenitors also form spheres and have been considered to expand only via expansion by their proliferation even from the single-cell level ( called spheres of pigment cells from the ciliary margin : PCM-spheres ) .
	manualset3
209958	7	418255	7	NULL	NULL	0	NULL	 expansion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinal stem/progenitor properties were also isolated from the ciliary body ( CB ) of the eye where , as in the CNS , such stem/progenitors also form spheres and have been considered to expand only via expansion by their proliferation even from the single-cell level ( called spheres of pigment cells from the ciliary margin : PCM-spheres ) .
	manualset3
209959	8	418255	7	NULL	NULL	0	NULL	proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinal stem/progenitor properties were also isolated from the ciliary body ( CB ) of the eye where , as in the CNS , such stem/progenitors also form spheres and have been considered to expand only via expansion by their proliferation even from the single-cell level ( called spheres of pigment cells from the ciliary margin : PCM-spheres ) .
	manualset3
209960	9	418255	7	NULL	NULL	0	NULL	single-cell level	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinal stem/progenitor properties were also isolated from the ciliary body ( CB ) of the eye where , as in the CNS , such stem/progenitors also form spheres and have been considered to expand only via expansion by their proliferation even from the single-cell level ( called spheres of pigment cells from the ciliary margin : PCM-spheres ) .
	manualset3
209961	10	418255	7	NULL	NULL	0	NULL	spheres	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinal stem/progenitor properties were also isolated from the ciliary body ( CB ) of the eye where , as in the CNS , such stem/progenitors also form spheres and have been considered to expand only via expansion by their proliferation even from the single-cell level ( called spheres of pigment cells from the ciliary margin : PCM-spheres ) .
	manualset3
209962	11	418255	7	NULL	NULL	0	NULL	pigment cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinal stem/progenitor properties were also isolated from the ciliary body ( CB ) of the eye where , as in the CNS , such stem/progenitors also form spheres and have been considered to expand only via expansion by their proliferation even from the single-cell level ( called spheres of pigment cells from the ciliary margin : PCM-spheres ) .
	manualset3
209963	12	418255	7	NULL	NULL	0	NULL	ciliary margin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinal stem/progenitor properties were also isolated from the ciliary body ( CB ) of the eye where , as in the CNS , such stem/progenitors also form spheres and have been considered to expand only via expansion by their proliferation even from the single-cell level ( called spheres of pigment cells from the ciliary margin : PCM-spheres ) .
	manualset3
209964	13	418255	7	NULL	NULL	0	NULL	PCM-spheres	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinal stem/progenitor properties were also isolated from the ciliary body ( CB ) of the eye where , as in the CNS , such stem/progenitors also form spheres and have been considered to expand only via expansion by their proliferation even from the single-cell level ( called spheres of pigment cells from the ciliary margin : PCM-spheres ) .
	manualset3
209965	1	418256	7	NULL	NULL	0	NULL	30 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Almost 30 % of the patients require corticosteroid treatment .
	manualset3
209966	2	418256	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Almost 30 % of the patients require corticosteroid treatment .
	manualset3
209967	3	418256	7	NULL	NULL	0	NULL	corticosteroid treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Almost 30 % of the patients require corticosteroid treatment .
	manualset3
209968	1	418257	7	NULL	NULL	0	NULL	118 , 9095 ( 2003 ) ) 	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	118 , 9095 ( 2003 ) ) can be interpreted as a two-parameter scaling of the zero order Hamiltonian , a generalization of the approach reported by Feenberg ( Phys .
	manualset3
209969	2	418257	7	NULL	NULL	0	NULL	two-parameter scaling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	118 , 9095 ( 2003 ) ) can be interpreted as a two-parameter scaling of the zero order Hamiltonian , a generalization of the approach reported by Feenberg ( Phys .
	manualset3
209970	3	418257	7	NULL	NULL	0	NULL	 zero order Hamiltonian	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	118 , 9095 ( 2003 ) ) can be interpreted as a two-parameter scaling of the zero order Hamiltonian , a generalization of the approach reported by Feenberg ( Phys .
	manualset3
209971	4	418257	7	NULL	NULL	0	NULL	generalization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	118 , 9095 ( 2003 ) ) can be interpreted as a two-parameter scaling of the zero order Hamiltonian , a generalization of the approach reported by Feenberg ( Phys .
	manualset3
209972	5	418257	7	NULL	NULL	0	NULL	 approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	118 , 9095 ( 2003 ) ) can be interpreted as a two-parameter scaling of the zero order Hamiltonian , a generalization of the approach reported by Feenberg ( Phys .
	manualset3
209973	6	418257	7	NULL	NULL	0	NULL	Feenberg ( Phys .	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	118 , 9095 ( 2003 ) ) can be interpreted as a two-parameter scaling of the zero order Hamiltonian , a generalization of the approach reported by Feenberg ( Phys .
	manualset3
209974	1	418258	7	NULL	NULL	0	NULL	Effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of atypical antipsychotics on weight and serum lipid levels .
	manualset3
209975	2	418258	7	NULL	NULL	0	NULL	atypical antipsychotics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of atypical antipsychotics on weight and serum lipid levels .
	manualset3
209976	3	418258	7	NULL	NULL	0	NULL	weight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of atypical antipsychotics on weight and serum lipid levels .
	manualset3
209977	4	418258	7	NULL	NULL	0	NULL	serum lipid levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of atypical antipsychotics on weight and serum lipid levels .
	manualset3
209978	1	418259	7	NULL	NULL	0	NULL	 responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Their responses were coded to make possible analysis by computer and were compared to responses from a national sample of dentists in the 1975 Survey of Dentists .
	manualset3
209979	2	418259	7	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Their responses were coded to make possible analysis by computer and were compared to responses from a national sample of dentists in the 1975 Survey of Dentists .
	manualset3
209980	3	418259	7	NULL	NULL	0	NULL	 computer	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Their responses were coded to make possible analysis by computer and were compared to responses from a national sample of dentists in the 1975 Survey of Dentists .
	manualset3
209981	4	418259	7	NULL	NULL	0	NULL	 responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Their responses were coded to make possible analysis by computer and were compared to responses from a national sample of dentists in the 1975 Survey of Dentists .
	manualset3
209982	5	418259	7	NULL	NULL	NULL	NULL	national sample of dentists	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Their responses were coded to make possible analysis by computer and were compared to responses from a national sample of dentists in the 1975 Survey of Dentists .
	manualset3
209983	6	418259	7	NULL	NULL	0	NULL	1975 Survey of Dentists	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Their responses were coded to make possible analysis by computer and were compared to responses from a national sample of dentists in the 1975 Survey of Dentists .
	manualset3
209984	1	418260	7	NULL	NULL	0	NULL	factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The factors that govern EpoR expression on the cell surface are poorly understood .
	manualset3
209985	2	418260	7	NULL	NULL	0	NULL	EpoR expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The factors that govern EpoR expression on the cell surface are poorly understood .
	manualset3
209986	3	418260	7	NULL	NULL	0	NULL	cell surface	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The factors that govern EpoR expression on the cell surface are poorly understood .
	manualset3
209987	1	418261	7	NULL	NULL	0	NULL	Fourty six per cent 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourty six per cent of the patients have stable iodine urine contents less or equal to 0.39 mumol/L .
	manualset3
209988	2	418261	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourty six per cent of the patients have stable iodine urine contents less or equal to 0.39 mumol/L .
	manualset3
209989	3	418261	7	NULL	NULL	0	NULL	iodine urine contents	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourty six per cent of the patients have stable iodine urine contents less or equal to 0.39 mumol/L .
	manualset3
209990	4	418261	7	NULL	NULL	0	NULL	0.39 mumol/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourty six per cent of the patients have stable iodine urine contents less or equal to 0.39 mumol/L .
	manualset3
209991	1	418262	7	NULL	NULL	0	NULL	Caries-inducing activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Caries-inducing activity of Palatinose syrup ) .
	manualset3
209992	2	418262	7	NULL	NULL	0	NULL	Palatinose syrup 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Caries-inducing activity of Palatinose syrup ) .
	manualset3
209993	1	418263	7	NULL	NULL	0	NULL	Integrated provirus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrated provirus was detected in all the chronic infections , including 0-47-1 in both cells .
	manualset3
209994	2	418263	7	NULL	NULL	0	NULL	chronic infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrated provirus was detected in all the chronic infections , including 0-47-1 in both cells .
	manualset3
209995	3	418263	7	NULL	NULL	0	NULL	0-47-1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrated provirus was detected in all the chronic infections , including 0-47-1 in both cells .
	manualset3
209996	4	418263	7	NULL	NULL	0	NULL	 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrated provirus was detected in all the chronic infections , including 0-47-1 in both cells .
	manualset3
209997	1	418264	7	NULL	NULL	0	NULL	catA gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The catA gene is approximately 3 kb from the catBC genes .
	manualset3
209998	2	418264	7	NULL	NULL	0	NULL	 3 kb	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The catA gene is approximately 3 kb from the catBC genes .
	manualset3
209999	3	418264	7	NULL	NULL	0	NULL	 catBC genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The catA gene is approximately 3 kb from the catBC genes .
	manualset3
210000	1	418265	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Unsurprisingly , when both the relationship characteristics and the health care context are appropriate there seems to be more positive outcomes for both nurse and client .
	manualset3
210001	2	418265	7	NULL	NULL	0	NULL	health care context	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Unsurprisingly , when both the relationship characteristics and the health care context are appropriate there seems to be more positive outcomes for both nurse and client .
	manualset3
210002	3	418265	7	NULL	NULL	0	NULL	 positive outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Unsurprisingly , when both the relationship characteristics and the health care context are appropriate there seems to be more positive outcomes for both nurse and client .
	manualset3
210003	4	418265	7	NULL	NULL	0	NULL	 nurse	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Unsurprisingly , when both the relationship characteristics and the health care context are appropriate there seems to be more positive outcomes for both nurse and client .
	manualset3
210004	5	418265	7	NULL	NULL	0	NULL	 client 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Unsurprisingly , when both the relationship characteristics and the health care context are appropriate there seems to be more positive outcomes for both nurse and client .
	manualset3
210005	1	418266	7	NULL	NULL	0	NULL	hemodialysis patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Almost all hemodialysis patients had HBeAg in their sera .
	manualset3
210006	2	418266	7	NULL	NULL	0	NULL	HBeAg	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Almost all hemodialysis patients had HBeAg in their sera .
	manualset3
210007	3	418266	7	NULL	NULL	0	NULL	sera	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Almost all hemodialysis patients had HBeAg in their sera .
	manualset3
210008	1	418267	7	NULL	NULL	0	NULL	essential therapeutic chance	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The essential therapeutic chance is offered by a firmly patterned ward structure and by creating an `` antidepressive environment '' which meets to a certain extent the patient 's innate craving for security and her need `` to belong '' , while at the same time promoting her own initiative and sense of responsibility .
	manualset3
210009	2	418267	7	NULL	NULL	0	NULL	firmly patterned ward structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The essential therapeutic chance is offered by a firmly patterned ward structure and by creating an `` antidepressive environment '' which meets to a certain extent the patient 's innate craving for security and her need `` to belong '' , while at the same time promoting her own initiative and sense of responsibility .
	manualset3
210010	3	418267	7	NULL	NULL	0	NULL	`` antidepressive environment ''	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The essential therapeutic chance is offered by a firmly patterned ward structure and by creating an `` antidepressive environment '' which meets to a certain extent the patient 's innate craving for security and her need `` to belong '' , while at the same time promoting her own initiative and sense of responsibility .
	manualset3
210011	4	418267	7	NULL	NULL	0	NULL	patient 's innate craving	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The essential therapeutic chance is offered by a firmly patterned ward structure and by creating an `` antidepressive environment '' which meets to a certain extent the patient 's innate craving for security and her need `` to belong '' , while at the same time promoting her own initiative and sense of responsibility .
	manualset3
210012	5	418267	7	NULL	NULL	0	NULL	security	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The essential therapeutic chance is offered by a firmly patterned ward structure and by creating an `` antidepressive environment '' which meets to a certain extent the patient 's innate craving for security and her need `` to belong '' , while at the same time promoting her own initiative and sense of responsibility .
	manualset3
210013	6	418267	7	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The essential therapeutic chance is offered by a firmly patterned ward structure and by creating an `` antidepressive environment '' which meets to a certain extent the patient 's innate craving for security and her need `` to belong '' , while at the same time promoting her own initiative and sense of responsibility .
	manualset3
210014	7	418267	7	NULL	NULL	0	NULL	sense of responsibility 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The essential therapeutic chance is offered by a firmly patterned ward structure and by creating an `` antidepressive environment '' which meets to a certain extent the patient 's innate craving for security and her need `` to belong '' , while at the same time promoting her own initiative and sense of responsibility .
	manualset3
210683	8	418267	7	NULL	NULL	0	NULL	initiative 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The essential therapeutic chance is offered by a firmly patterned ward structure and by creating an `` antidepressive environment '' which meets to a certain extent the patient 's innate craving for security and her need `` to belong '' , while at the same time promoting her own initiative and sense of responsibility .
	manualset3
210015	1	418268	7	NULL	NULL	0	NULL	Surgical therapies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Surgical therapies in brain metastasis .
	manualset3
210016	2	418268	7	NULL	NULL	0	NULL	brain metastasis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Surgical therapies in brain metastasis .
	manualset3
210017	1	418269	7	NULL	NULL	0	NULL	Measurement 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of Fru ( 2 , 6 ) P2 proved to be the most sensitive parameter for an assessment of glycolysis : IL1 alpha , IL1 beta and IFN-gamma all produced a 3-6-fold increase in this metabolite whereas tumor necrosis factor ( TNF alpha ) was far less effective .
	manualset3
210018	2	418269	7	NULL	NULL	0	NULL	Fru ( 2 , 6 ) P2	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of Fru ( 2 , 6 ) P2 proved to be the most sensitive parameter for an assessment of glycolysis : IL1 alpha , IL1 beta and IFN-gamma all produced a 3-6-fold increase in this metabolite whereas tumor necrosis factor ( TNF alpha ) was far less effective .
	manualset3
210019	3	418269	7	NULL	NULL	0	NULL	sensitive parameter	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of Fru ( 2 , 6 ) P2 proved to be the most sensitive parameter for an assessment of glycolysis : IL1 alpha , IL1 beta and IFN-gamma all produced a 3-6-fold increase in this metabolite whereas tumor necrosis factor ( TNF alpha ) was far less effective .
	manualset3
210020	4	418269	7	NULL	NULL	0	NULL	 assessment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of Fru ( 2 , 6 ) P2 proved to be the most sensitive parameter for an assessment of glycolysis : IL1 alpha , IL1 beta and IFN-gamma all produced a 3-6-fold increase in this metabolite whereas tumor necrosis factor ( TNF alpha ) was far less effective .
	manualset3
210021	5	418269	7	NULL	NULL	0	NULL	glycolysis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of Fru ( 2 , 6 ) P2 proved to be the most sensitive parameter for an assessment of glycolysis : IL1 alpha , IL1 beta and IFN-gamma all produced a 3-6-fold increase in this metabolite whereas tumor necrosis factor ( TNF alpha ) was far less effective .
	manualset3
210022	6	418269	7	NULL	NULL	0	NULL	IL1 alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of Fru ( 2 , 6 ) P2 proved to be the most sensitive parameter for an assessment of glycolysis : IL1 alpha , IL1 beta and IFN-gamma all produced a 3-6-fold increase in this metabolite whereas tumor necrosis factor ( TNF alpha ) was far less effective .
	manualset3
210023	7	418269	7	NULL	NULL	0	NULL	IL1 beta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of Fru ( 2 , 6 ) P2 proved to be the most sensitive parameter for an assessment of glycolysis : IL1 alpha , IL1 beta and IFN-gamma all produced a 3-6-fold increase in this metabolite whereas tumor necrosis factor ( TNF alpha ) was far less effective .
	manualset3
210024	8	418269	7	NULL	NULL	0	NULL	IFN-gamma	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of Fru ( 2 , 6 ) P2 proved to be the most sensitive parameter for an assessment of glycolysis : IL1 alpha , IL1 beta and IFN-gamma all produced a 3-6-fold increase in this metabolite whereas tumor necrosis factor ( TNF alpha ) was far less effective .
	manualset3
210025	9	418269	7	NULL	NULL	0	NULL	3-6-fold increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of Fru ( 2 , 6 ) P2 proved to be the most sensitive parameter for an assessment of glycolysis : IL1 alpha , IL1 beta and IFN-gamma all produced a 3-6-fold increase in this metabolite whereas tumor necrosis factor ( TNF alpha ) was far less effective .
	manualset3
210026	10	418269	7	NULL	NULL	0	NULL	metabolite	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of Fru ( 2 , 6 ) P2 proved to be the most sensitive parameter for an assessment of glycolysis : IL1 alpha , IL1 beta and IFN-gamma all produced a 3-6-fold increase in this metabolite whereas tumor necrosis factor ( TNF alpha ) was far less effective .
	manualset3
210027	11	418269	7	NULL	NULL	0	NULL	 tumor necrosis factor ( TNF alpha )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of Fru ( 2 , 6 ) P2 proved to be the most sensitive parameter for an assessment of glycolysis : IL1 alpha , IL1 beta and IFN-gamma all produced a 3-6-fold increase in this metabolite whereas tumor necrosis factor ( TNF alpha ) was far less effective .
	manualset3
210028	1	418270	7	NULL	NULL	0	NULL	Mutation analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation analysis led to the conclusion that pauA3B2 participate in catabolism of DAP , which is related to the aminopropyl moiety of Spd , and that bauABCD are essential for growth on - alanine derived from DAP ( or Spd ) catabolism via the - glutamylation pathway .
	manualset3
210029	2	418270	7	NULL	NULL	0	NULL	 conclusion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation analysis led to the conclusion that pauA3B2 participate in catabolism of DAP , which is related to the aminopropyl moiety of Spd , and that bauABCD are essential for growth on - alanine derived from DAP ( or Spd ) catabolism via the - glutamylation pathway .
	manualset3
210030	3	418270	7	NULL	NULL	0	NULL	pauA3B2	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation analysis led to the conclusion that pauA3B2 participate in catabolism of DAP , which is related to the aminopropyl moiety of Spd , and that bauABCD are essential for growth on - alanine derived from DAP ( or Spd ) catabolism via the - glutamylation pathway .
	manualset3
210031	4	418270	7	NULL	NULL	0	NULL	 catabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation analysis led to the conclusion that pauA3B2 participate in catabolism of DAP , which is related to the aminopropyl moiety of Spd , and that bauABCD are essential for growth on - alanine derived from DAP ( or Spd ) catabolism via the - glutamylation pathway .
	manualset3
210032	5	418270	7	NULL	NULL	0	NULL	DAP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation analysis led to the conclusion that pauA3B2 participate in catabolism of DAP , which is related to the aminopropyl moiety of Spd , and that bauABCD are essential for growth on - alanine derived from DAP ( or Spd ) catabolism via the - glutamylation pathway .
	manualset3
210033	6	418270	7	NULL	NULL	0	NULL	aminopropyl moiety	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation analysis led to the conclusion that pauA3B2 participate in catabolism of DAP , which is related to the aminopropyl moiety of Spd , and that bauABCD are essential for growth on - alanine derived from DAP ( or Spd ) catabolism via the - glutamylation pathway .
	manualset3
210034	7	418270	7	NULL	NULL	0	NULL	 Spd	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation analysis led to the conclusion that pauA3B2 participate in catabolism of DAP , which is related to the aminopropyl moiety of Spd , and that bauABCD are essential for growth on - alanine derived from DAP ( or Spd ) catabolism via the - glutamylation pathway .
	manualset3
210035	8	418270	7	NULL	NULL	0	NULL	bauABCD	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation analysis led to the conclusion that pauA3B2 participate in catabolism of DAP , which is related to the aminopropyl moiety of Spd , and that bauABCD are essential for growth on - alanine derived from DAP ( or Spd ) catabolism via the - glutamylation pathway .
	manualset3
210036	9	418270	7	NULL	NULL	0	NULL	growth	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation analysis led to the conclusion that pauA3B2 participate in catabolism of DAP , which is related to the aminopropyl moiety of Spd , and that bauABCD are essential for growth on - alanine derived from DAP ( or Spd ) catabolism via the - glutamylation pathway .
	manualset3
210037	10	418270	7	NULL	NULL	0	NULL	alanine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation analysis led to the conclusion that pauA3B2 participate in catabolism of DAP , which is related to the aminopropyl moiety of Spd , and that bauABCD are essential for growth on - alanine derived from DAP ( or Spd ) catabolism via the - glutamylation pathway .
	manualset3
210038	11	418270	7	NULL	NULL	0	NULL	 DAP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation analysis led to the conclusion that pauA3B2 participate in catabolism of DAP , which is related to the aminopropyl moiety of Spd , and that bauABCD are essential for growth on - alanine derived from DAP ( or Spd ) catabolism via the - glutamylation pathway .
	manualset3
210039	12	418270	7	NULL	NULL	0	NULL	Spd 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation analysis led to the conclusion that pauA3B2 participate in catabolism of DAP , which is related to the aminopropyl moiety of Spd , and that bauABCD are essential for growth on - alanine derived from DAP ( or Spd ) catabolism via the - glutamylation pathway .
	manualset3
210040	13	418270	7	NULL	NULL	0	NULL	catabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation analysis led to the conclusion that pauA3B2 participate in catabolism of DAP , which is related to the aminopropyl moiety of Spd , and that bauABCD are essential for growth on - alanine derived from DAP ( or Spd ) catabolism via the - glutamylation pathway .
	manualset3
210041	14	418270	7	NULL	NULL	0	NULL	 glutamylation pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutation analysis led to the conclusion that pauA3B2 participate in catabolism of DAP , which is related to the aminopropyl moiety of Spd , and that bauABCD are essential for growth on - alanine derived from DAP ( or Spd ) catabolism via the - glutamylation pathway .
	manualset3
210042	1	418271	7	NULL	NULL	0	NULL	170 primary invasive carcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In 170 primary invasive carcinomas of the breast , morphological criteria of the primary tumor -- tumor size , WHO classification , malignancy according to Bloom , number and status of foci , lymphangiosis carcinomatosa , stroma reaction -- were compared with the axillary lymph node status .
	manualset3
210043	2	418271	7	NULL	NULL	0	NULL	breast	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In 170 primary invasive carcinomas of the breast , morphological criteria of the primary tumor -- tumor size , WHO classification , malignancy according to Bloom , number and status of foci , lymphangiosis carcinomatosa , stroma reaction -- were compared with the axillary lymph node status .
	manualset3
210044	3	418271	7	NULL	NULL	0	NULL	morphological criteria	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In 170 primary invasive carcinomas of the breast , morphological criteria of the primary tumor -- tumor size , WHO classification , malignancy according to Bloom , number and status of foci , lymphangiosis carcinomatosa , stroma reaction -- were compared with the axillary lymph node status .
	manualset3
210045	4	418271	7	NULL	NULL	0	NULL	primary tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 170 primary invasive carcinomas of the breast , morphological criteria of the primary tumor -- tumor size , WHO classification , malignancy according to Bloom , number and status of foci , lymphangiosis carcinomatosa , stroma reaction -- were compared with the axillary lymph node status .
	manualset3
210046	5	418271	7	NULL	NULL	0	NULL	tumor size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 170 primary invasive carcinomas of the breast , morphological criteria of the primary tumor -- tumor size , WHO classification , malignancy according to Bloom , number and status of foci , lymphangiosis carcinomatosa , stroma reaction -- were compared with the axillary lymph node status .
	manualset3
210047	6	418271	7	NULL	NULL	0	NULL	WHO classification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In 170 primary invasive carcinomas of the breast , morphological criteria of the primary tumor -- tumor size , WHO classification , malignancy according to Bloom , number and status of foci , lymphangiosis carcinomatosa , stroma reaction -- were compared with the axillary lymph node status .
	manualset3
210048	7	418271	7	NULL	NULL	0	NULL	malignancy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In 170 primary invasive carcinomas of the breast , morphological criteria of the primary tumor -- tumor size , WHO classification , malignancy according to Bloom , number and status of foci , lymphangiosis carcinomatosa , stroma reaction -- were compared with the axillary lymph node status .
	manualset3
210049	8	418271	7	NULL	NULL	0	NULL	Bloom	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 170 primary invasive carcinomas of the breast , morphological criteria of the primary tumor -- tumor size , WHO classification , malignancy according to Bloom , number and status of foci , lymphangiosis carcinomatosa , stroma reaction -- were compared with the axillary lymph node status .
	manualset3
210050	9	418271	7	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 170 primary invasive carcinomas of the breast , morphological criteria of the primary tumor -- tumor size , WHO classification , malignancy according to Bloom , number and status of foci , lymphangiosis carcinomatosa , stroma reaction -- were compared with the axillary lymph node status .
	manualset3
210051	10	418271	7	NULL	NULL	0	NULL	 status of foci 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In 170 primary invasive carcinomas of the breast , morphological criteria of the primary tumor -- tumor size , WHO classification , malignancy according to Bloom , number and status of foci , lymphangiosis carcinomatosa , stroma reaction -- were compared with the axillary lymph node status .
	manualset3
210052	11	418271	7	NULL	NULL	0	NULL	lymphangiosis carcinomatosa	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In 170 primary invasive carcinomas of the breast , morphological criteria of the primary tumor -- tumor size , WHO classification , malignancy according to Bloom , number and status of foci , lymphangiosis carcinomatosa , stroma reaction -- were compared with the axillary lymph node status .
	manualset3
210053	12	418271	7	NULL	NULL	0	NULL	stroma reaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In 170 primary invasive carcinomas of the breast , morphological criteria of the primary tumor -- tumor size , WHO classification , malignancy according to Bloom , number and status of foci , lymphangiosis carcinomatosa , stroma reaction -- were compared with the axillary lymph node status .
	manualset3
210054	13	418271	7	NULL	NULL	0	NULL	axillary lymph node status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 170 primary invasive carcinomas of the breast , morphological criteria of the primary tumor -- tumor size , WHO classification , malignancy according to Bloom , number and status of foci , lymphangiosis carcinomatosa , stroma reaction -- were compared with the axillary lymph node status .
	manualset3
210055	1	418272	7	NULL	NULL	0	NULL	Doxorubicin ( Dox ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Doxorubicin ( Dox ) is known to cause cardiomyopathy and congestive heart failure upon chronic administration .
	manualset3
210056	2	418272	7	NULL	NULL	0	NULL	cardiomyopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Doxorubicin ( Dox ) is known to cause cardiomyopathy and congestive heart failure upon chronic administration .
	manualset3
210057	3	418272	7	NULL	NULL	0	NULL	congestive heart failure	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Doxorubicin ( Dox ) is known to cause cardiomyopathy and congestive heart failure upon chronic administration .
	manualset3
210058	4	418272	7	NULL	NULL	0	NULL	 chronic administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Doxorubicin ( Dox ) is known to cause cardiomyopathy and congestive heart failure upon chronic administration .
	manualset3
210059	1	418273	7	NULL	NULL	0	NULL	Systemic hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Systemic hypertension and anesthesia . ) .
	manualset3
210060	2	418273	7	NULL	NULL	0	NULL	 anesthesia	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Systemic hypertension and anesthesia . ) .
	manualset3
210061	1	418274	7	NULL	NULL	0	NULL	Subclinical pulmonary dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Subclinical pulmonary dysfunction : an unrecognized diabetes complication ? ) .
	manualset3
210062	2	418274	7	NULL	NULL	0	NULL	unrecognized diabetes complication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Subclinical pulmonary dysfunction : an unrecognized diabetes complication ? ) .
	manualset3
210063	1	418275	7	NULL	NULL	0	NULL	applications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The applications of this approach in the fringe pattern analyses are also introduced .
	manualset3
210064	2	418275	7	NULL	NULL	0	NULL	approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The applications of this approach in the fringe pattern analyses are also introduced .
	manualset3
210065	3	418275	7	NULL	NULL	0	NULL	fringe pattern analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The applications of this approach in the fringe pattern analyses are also introduced .
	manualset3
210066	1	418276	7	NULL	NULL	0	NULL	Patterns	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patterns of major lifestyle behaviors associated with cardiovascular disease are established early in childhood and influence risk factors for cardiovascular disease in childhood and adolescence as well as in adulthood .
	manualset3
210067	2	418276	7	NULL	NULL	0	NULL	major lifestyle behaviors	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Patterns of major lifestyle behaviors associated with cardiovascular disease are established early in childhood and influence risk factors for cardiovascular disease in childhood and adolescence as well as in adulthood .
	manualset3
210068	3	418276	7	NULL	NULL	0	NULL	cardiovascular disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patterns of major lifestyle behaviors associated with cardiovascular disease are established early in childhood and influence risk factors for cardiovascular disease in childhood and adolescence as well as in adulthood .
	manualset3
210069	4	418276	7	NULL	NULL	0	NULL	childhood	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Patterns of major lifestyle behaviors associated with cardiovascular disease are established early in childhood and influence risk factors for cardiovascular disease in childhood and adolescence as well as in adulthood .
	manualset3
210070	5	418276	7	NULL	NULL	0	NULL	 risk factors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patterns of major lifestyle behaviors associated with cardiovascular disease are established early in childhood and influence risk factors for cardiovascular disease in childhood and adolescence as well as in adulthood .
	manualset3
210071	6	418276	7	NULL	NULL	0	NULL	cardiovascular disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patterns of major lifestyle behaviors associated with cardiovascular disease are established early in childhood and influence risk factors for cardiovascular disease in childhood and adolescence as well as in adulthood .
	manualset3
210072	7	418276	7	NULL	NULL	0	NULL	childhood	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Patterns of major lifestyle behaviors associated with cardiovascular disease are established early in childhood and influence risk factors for cardiovascular disease in childhood and adolescence as well as in adulthood .
	manualset3
210073	8	418276	7	NULL	NULL	0	NULL	adolescence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Patterns of major lifestyle behaviors associated with cardiovascular disease are established early in childhood and influence risk factors for cardiovascular disease in childhood and adolescence as well as in adulthood .
	manualset3
210074	9	418276	7	NULL	NULL	0	NULL	 adulthood 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Patterns of major lifestyle behaviors associated with cardiovascular disease are established early in childhood and influence risk factors for cardiovascular disease in childhood and adolescence as well as in adulthood .
	manualset3
210075	1	418277	7	NULL	NULL	0	NULL	 end-tidal enflurane concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The end-tidal enflurane concentration was held constant for 25-36 min in order to equilibrate the brain with the alveolar anasthetic partial pressure .
	manualset3
210076	2	418277	7	NULL	NULL	0	NULL	 25-36 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The end-tidal enflurane concentration was held constant for 25-36 min in order to equilibrate the brain with the alveolar anasthetic partial pressure .
	manualset3
210077	3	418277	7	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The end-tidal enflurane concentration was held constant for 25-36 min in order to equilibrate the brain with the alveolar anasthetic partial pressure .
	manualset3
210078	4	418277	7	NULL	NULL	0	NULL	 alveolar anasthetic partial pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The end-tidal enflurane concentration was held constant for 25-36 min in order to equilibrate the brain with the alveolar anasthetic partial pressure .
	manualset3
210079	1	418278	7	NULL	NULL	0	NULL	Results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that ADCC contributes to killing of CLL cells by anti-CD20 antibodies ( rituximab and veltuzumab ) , whereas mAbs against CD22 ( epratuzumab ) and CD23 ( lumiliximab ) showed minimal ADCC .
	manualset3
210080	2	418278	7	NULL	NULL	0	NULL	ADCC	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that ADCC contributes to killing of CLL cells by anti-CD20 antibodies ( rituximab and veltuzumab ) , whereas mAbs against CD22 ( epratuzumab ) and CD23 ( lumiliximab ) showed minimal ADCC .
	manualset3
210081	3	418278	7	NULL	NULL	0	NULL	CLL cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that ADCC contributes to killing of CLL cells by anti-CD20 antibodies ( rituximab and veltuzumab ) , whereas mAbs against CD22 ( epratuzumab ) and CD23 ( lumiliximab ) showed minimal ADCC .
	manualset3
210082	4	418278	7	NULL	NULL	0	NULL	anti-CD20 antibodies	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that ADCC contributes to killing of CLL cells by anti-CD20 antibodies ( rituximab and veltuzumab ) , whereas mAbs against CD22 ( epratuzumab ) and CD23 ( lumiliximab ) showed minimal ADCC .
	manualset3
210083	5	418278	7	NULL	NULL	0	NULL	rituximab	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that ADCC contributes to killing of CLL cells by anti-CD20 antibodies ( rituximab and veltuzumab ) , whereas mAbs against CD22 ( epratuzumab ) and CD23 ( lumiliximab ) showed minimal ADCC .
	manualset3
210084	6	418278	7	NULL	NULL	0	NULL	 veltuzumab	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that ADCC contributes to killing of CLL cells by anti-CD20 antibodies ( rituximab and veltuzumab ) , whereas mAbs against CD22 ( epratuzumab ) and CD23 ( lumiliximab ) showed minimal ADCC .
	manualset3
210085	7	418278	7	NULL	NULL	0	NULL	mAbs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that ADCC contributes to killing of CLL cells by anti-CD20 antibodies ( rituximab and veltuzumab ) , whereas mAbs against CD22 ( epratuzumab ) and CD23 ( lumiliximab ) showed minimal ADCC .
	manualset3
210086	8	418278	7	NULL	NULL	0	NULL	CD22	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that ADCC contributes to killing of CLL cells by anti-CD20 antibodies ( rituximab and veltuzumab ) , whereas mAbs against CD22 ( epratuzumab ) and CD23 ( lumiliximab ) showed minimal ADCC .
	manualset3
210087	9	418278	7	NULL	NULL	0	NULL	epratuzumab	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that ADCC contributes to killing of CLL cells by anti-CD20 antibodies ( rituximab and veltuzumab ) , whereas mAbs against CD22 ( epratuzumab ) and CD23 ( lumiliximab ) showed minimal ADCC .
	manualset3
210088	10	418278	7	NULL	NULL	0	NULL	CD23	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that ADCC contributes to killing of CLL cells by anti-CD20 antibodies ( rituximab and veltuzumab ) , whereas mAbs against CD22 ( epratuzumab ) and CD23 ( lumiliximab ) showed minimal ADCC .
	manualset3
210089	11	418278	7	NULL	NULL	0	NULL	lumiliximab	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that ADCC contributes to killing of CLL cells by anti-CD20 antibodies ( rituximab and veltuzumab ) , whereas mAbs against CD22 ( epratuzumab ) and CD23 ( lumiliximab ) showed minimal ADCC .
	manualset3
210090	12	418278	7	NULL	NULL	0	NULL	minimal ADCC	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest that ADCC contributes to killing of CLL cells by anti-CD20 antibodies ( rituximab and veltuzumab ) , whereas mAbs against CD22 ( epratuzumab ) and CD23 ( lumiliximab ) showed minimal ADCC .
	manualset3
210091	1	418279	7	NULL	NULL	0	NULL	RRFs 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Almost all RRFs showed sarcoplasmic expression of XIAP .
	manualset3
210092	2	418279	7	NULL	NULL	0	NULL	sarcoplasmic expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Almost all RRFs showed sarcoplasmic expression of XIAP .
	manualset3
210093	3	418279	7	NULL	NULL	0	NULL	XIAP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Almost all RRFs showed sarcoplasmic expression of XIAP .
	manualset3
210094	1	418280	7	NULL	NULL	0	NULL	Artificial ripening	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Artificial ripening of the cervix by local action of maternal leukocytes ) .
	manualset3
210095	2	418280	7	NULL	NULL	0	NULL	cervix 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Artificial ripening of the cervix by local action of maternal leukocytes ) .
	manualset3
210096	3	418280	7	NULL	NULL	0	NULL	local action	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Artificial ripening of the cervix by local action of maternal leukocytes ) .
	manualset3
210097	4	418280	7	NULL	NULL	0	NULL	maternal leukocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	( Artificial ripening of the cervix by local action of maternal leukocytes ) .
	manualset3
210098	1	418281	7	NULL	NULL	0	NULL	BDJ	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Now , before the BDJ is bombarded with complaints about ivory-tower academics talking theoretically about something of which they have no experience , I need to tell you that I do have real , live practical experience of business .
	manualset3
210099	2	418281	7	NULL	NULL	0	NULL	complaints	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Now , before the BDJ is bombarded with complaints about ivory-tower academics talking theoretically about something of which they have no experience , I need to tell you that I do have real , live practical experience of business .
	manualset3
210100	3	418281	7	NULL	NULL	0	NULL	ivory-tower academics	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Now , before the BDJ is bombarded with complaints about ivory-tower academics talking theoretically about something of which they have no experience , I need to tell you that I do have real , live practical experience of business .
	manualset3
210101	4	418281	7	NULL	NULL	0	NULL	experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Now , before the BDJ is bombarded with complaints about ivory-tower academics talking theoretically about something of which they have no experience , I need to tell you that I do have real , live practical experience of business .
	manualset3
210102	5	418281	7	NULL	NULL	0	NULL	real , live practical experience 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Now , before the BDJ is bombarded with complaints about ivory-tower academics talking theoretically about something of which they have no experience , I need to tell you that I do have real , live practical experience of business .
	manualset3
210103	6	418281	7	NULL	NULL	0	NULL	business	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Now , before the BDJ is bombarded with complaints about ivory-tower academics talking theoretically about something of which they have no experience , I need to tell you that I do have real , live practical experience of business .
	manualset3
210104	1	418282	7	NULL	NULL	0	NULL	gestational age	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although premature , and small for gestational age , he had a normal growth , and did not show any clinical sign suggestive of immune deficiency .
	manualset3
210105	2	418282	7	NULL	NULL	0	NULL	 normal growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although premature , and small for gestational age , he had a normal growth , and did not show any clinical sign suggestive of immune deficiency .
	manualset3
210106	3	418282	7	NULL	NULL	0	NULL	clinical sign	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although premature , and small for gestational age , he had a normal growth , and did not show any clinical sign suggestive of immune deficiency .
	manualset3
210107	4	418282	7	NULL	NULL	0	NULL	 immune deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although premature , and small for gestational age , he had a normal growth , and did not show any clinical sign suggestive of immune deficiency .
	manualset3
210108	1	418283	7	NULL	NULL	0	NULL	Single-cell microbeam irradiators	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-cell microbeam irradiators are of increasing interest to the biological community .
	manualset3
210109	2	418283	7	NULL	NULL	0	NULL	 biological community 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-cell microbeam irradiators are of increasing interest to the biological community .
	manualset3
210110	1	418284	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show for the first time that E2 , estrone , DES and TAM can be activated by DMDO and possibly to epoxides .
	manualset3
210111	2	418284	7	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show for the first time that E2 , estrone , DES and TAM can be activated by DMDO and possibly to epoxides .
	manualset3
210112	3	418284	7	NULL	NULL	0	NULL	E2	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show for the first time that E2 , estrone , DES and TAM can be activated by DMDO and possibly to epoxides .
	manualset3
210113	4	418284	7	NULL	NULL	0	NULL	estrone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show for the first time that E2 , estrone , DES and TAM can be activated by DMDO and possibly to epoxides .
	manualset3
210114	5	418284	7	NULL	NULL	0	NULL	DES	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show for the first time that E2 , estrone , DES and TAM can be activated by DMDO and possibly to epoxides .
	manualset3
210115	6	418284	7	NULL	NULL	0	NULL	TAM	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show for the first time that E2 , estrone , DES and TAM can be activated by DMDO and possibly to epoxides .
	manualset3
210116	7	418284	7	NULL	NULL	0	NULL	DMDO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show for the first time that E2 , estrone , DES and TAM can be activated by DMDO and possibly to epoxides .
	manualset3
210117	8	418284	7	NULL	NULL	0	NULL	epoxides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data show for the first time that E2 , estrone , DES and TAM can be activated by DMDO and possibly to epoxides .
	manualset3
210118	1	418285	7	NULL	NULL	0	NULL	Management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Management of inflammatory breast cancer after neo-adjuvant chemotherapy ) .
	manualset3
210119	2	418285	7	NULL	NULL	0	NULL	inflammatory breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Management of inflammatory breast cancer after neo-adjuvant chemotherapy ) .
	manualset3
210120	3	418285	7	NULL	NULL	0	NULL	neo-adjuvant chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Management of inflammatory breast cancer after neo-adjuvant chemotherapy ) .
	manualset3
210121	1	418286	7	NULL	NULL	0	NULL	Cm ( III )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We chose Cm ( III ) due to its high fluorescence spectroscopic sensitivity as a model system for exploring the interactions of trivalent actinides with D. spensis in the trace concentration range of 3 x 10 ( -7 ) mol/L .
	manualset3
210122	2	418286	7	NULL	NULL	0	NULL	high fluorescence spectroscopic sensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We chose Cm ( III ) due to its high fluorescence spectroscopic sensitivity as a model system for exploring the interactions of trivalent actinides with D. spensis in the trace concentration range of 3 x 10 ( -7 ) mol/L .
	manualset3
210123	3	418286	7	NULL	NULL	0	NULL	 model system	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We chose Cm ( III ) due to its high fluorescence spectroscopic sensitivity as a model system for exploring the interactions of trivalent actinides with D. spensis in the trace concentration range of 3 x 10 ( -7 ) mol/L .
	manualset3
210124	4	418286	7	NULL	NULL	0	NULL	interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We chose Cm ( III ) due to its high fluorescence spectroscopic sensitivity as a model system for exploring the interactions of trivalent actinides with D. spensis in the trace concentration range of 3 x 10 ( -7 ) mol/L .
	manualset3
210125	5	418286	7	NULL	NULL	0	NULL	trivalent actinides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We chose Cm ( III ) due to its high fluorescence spectroscopic sensitivity as a model system for exploring the interactions of trivalent actinides with D. spensis in the trace concentration range of 3 x 10 ( -7 ) mol/L .
	manualset3
210126	6	418286	7	NULL	NULL	0	NULL	D. spensis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We chose Cm ( III ) due to its high fluorescence spectroscopic sensitivity as a model system for exploring the interactions of trivalent actinides with D. spensis in the trace concentration range of 3 x 10 ( -7 ) mol/L .
	manualset3
210127	7	418286	7	NULL	NULL	0	NULL	trace concentration range 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We chose Cm ( III ) due to its high fluorescence spectroscopic sensitivity as a model system for exploring the interactions of trivalent actinides with D. spensis in the trace concentration range of 3 x 10 ( -7 ) mol/L .
	manualset3
210128	8	418286	7	NULL	NULL	0	NULL	 3 x 10 ( -7 ) mol/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	We chose Cm ( III ) due to its high fluorescence spectroscopic sensitivity as a model system for exploring the interactions of trivalent actinides with D. spensis in the trace concentration range of 3 x 10 ( -7 ) mol/L .
	manualset3
210129	1	418287	7	NULL	NULL	0	NULL	Seven days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven days after nerve transection the regenerating structure within the chamber consisted primarily of a fibrous matrix which stained with anti-fibronectin but not anti-laminin .
	manualset3
210130	2	418287	7	NULL	NULL	0	NULL	nerve transection	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven days after nerve transection the regenerating structure within the chamber consisted primarily of a fibrous matrix which stained with anti-fibronectin but not anti-laminin .
	manualset3
210131	3	418287	7	NULL	NULL	0	NULL	regenerating structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven days after nerve transection the regenerating structure within the chamber consisted primarily of a fibrous matrix which stained with anti-fibronectin but not anti-laminin .
	manualset3
210132	4	418287	7	NULL	NULL	0	NULL	chamber	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven days after nerve transection the regenerating structure within the chamber consisted primarily of a fibrous matrix which stained with anti-fibronectin but not anti-laminin .
	manualset3
210133	5	418287	7	NULL	NULL	0	NULL	fibrous matrix	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven days after nerve transection the regenerating structure within the chamber consisted primarily of a fibrous matrix which stained with anti-fibronectin but not anti-laminin .
	manualset3
210134	6	418287	7	NULL	NULL	0	NULL	anti-fibronectin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven days after nerve transection the regenerating structure within the chamber consisted primarily of a fibrous matrix which stained with anti-fibronectin but not anti-laminin .
	manualset3
210135	7	418287	7	NULL	NULL	0	NULL	anti-laminin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven days after nerve transection the regenerating structure within the chamber consisted primarily of a fibrous matrix which stained with anti-fibronectin but not anti-laminin .
	manualset3
210136	1	418288	7	NULL	NULL	0	NULL	Four 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four of the 50 serum samples from mares affected with CEM showed PHA titers of 1 : 32 , while most of the samples ( 92.0 % ) showed PHA titers greater than 1 : 32 .
	manualset3
210137	2	418288	7	NULL	NULL	0	NULL	50 serum samples	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Four of the 50 serum samples from mares affected with CEM showed PHA titers of 1 : 32 , while most of the samples ( 92.0 % ) showed PHA titers greater than 1 : 32 .
	manualset3
210138	3	418288	7	NULL	NULL	0	NULL	mares	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Four of the 50 serum samples from mares affected with CEM showed PHA titers of 1 : 32 , while most of the samples ( 92.0 % ) showed PHA titers greater than 1 : 32 .
	manualset3
210139	4	418288	7	NULL	NULL	0	NULL	CEM	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Four of the 50 serum samples from mares affected with CEM showed PHA titers of 1 : 32 , while most of the samples ( 92.0 % ) showed PHA titers greater than 1 : 32 .
	manualset3
210140	5	418288	7	NULL	NULL	0	NULL	PHA titers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four of the 50 serum samples from mares affected with CEM showed PHA titers of 1 : 32 , while most of the samples ( 92.0 % ) showed PHA titers greater than 1 : 32 .
	manualset3
210141	6	418288	7	NULL	NULL	0	NULL	1 : 32	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four of the 50 serum samples from mares affected with CEM showed PHA titers of 1 : 32 , while most of the samples ( 92.0 % ) showed PHA titers greater than 1 : 32 .
	manualset3
210142	7	418288	7	NULL	NULL	0	NULL	samples	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Four of the 50 serum samples from mares affected with CEM showed PHA titers of 1 : 32 , while most of the samples ( 92.0 % ) showed PHA titers greater than 1 : 32 .
	manualset3
210143	8	418288	7	NULL	NULL	0	NULL	 92.0 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four of the 50 serum samples from mares affected with CEM showed PHA titers of 1 : 32 , while most of the samples ( 92.0 % ) showed PHA titers greater than 1 : 32 .
	manualset3
210144	9	418288	7	NULL	NULL	0	NULL	PHA titers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four of the 50 serum samples from mares affected with CEM showed PHA titers of 1 : 32 , while most of the samples ( 92.0 % ) showed PHA titers greater than 1 : 32 .
	manualset3
210145	10	418288	7	NULL	NULL	0	NULL	1 : 32	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four of the 50 serum samples from mares affected with CEM showed PHA titers of 1 : 32 , while most of the samples ( 92.0 % ) showed PHA titers greater than 1 : 32 .
	manualset3
210146	1	418289	7	NULL	NULL	NULL	NULL	distribution 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The distribution of soluble Kit levels was investigated among 112 normal human serum donors .
	manualset3
210147	2	418289	7	NULL	NULL	0	NULL	soluble Kit levels	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of soluble Kit levels was investigated among 112 normal human serum donors .
	manualset3
210148	3	418289	7	NULL	NULL	0	NULL	112 normal human serum donors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The distribution of soluble Kit levels was investigated among 112 normal human serum donors .
	manualset3
210149	1	418290	7	NULL	NULL	0	NULL	poly-D-lysine/laminin plates	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro , using poly-D-lysine/laminin plates , KRAS mutant cell lines were resistant to cetuximab , whereas KRAS wild-type lines showed sensitivity to cetuximab .
	manualset3
210150	2	418290	7	NULL	NULL	0	NULL	KRAS mutant cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro , using poly-D-lysine/laminin plates , KRAS mutant cell lines were resistant to cetuximab , whereas KRAS wild-type lines showed sensitivity to cetuximab .
	manualset3
210151	3	418290	7	NULL	NULL	0	NULL	cetuximab	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro , using poly-D-lysine/laminin plates , KRAS mutant cell lines were resistant to cetuximab , whereas KRAS wild-type lines showed sensitivity to cetuximab .
	manualset3
210152	4	418290	7	NULL	NULL	0	NULL	KRAS wild-type lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro , using poly-D-lysine/laminin plates , KRAS mutant cell lines were resistant to cetuximab , whereas KRAS wild-type lines showed sensitivity to cetuximab .
	manualset3
210153	5	418290	7	NULL	NULL	0	NULL	sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro , using poly-D-lysine/laminin plates , KRAS mutant cell lines were resistant to cetuximab , whereas KRAS wild-type lines showed sensitivity to cetuximab .
	manualset3
210154	6	418290	7	NULL	NULL	0	NULL	cetuximab	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro , using poly-D-lysine/laminin plates , KRAS mutant cell lines were resistant to cetuximab , whereas KRAS wild-type lines showed sensitivity to cetuximab .
	manualset3
210155	1	418291	7	NULL	NULL	0	NULL	variation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The variation in the degree of abnormality found in dizygotic twins exposed to similar amounts of alcohol at the same time during gestation indicates that differences in fetal susceptibility to ethanol dysmorphogenesis are of prime importance to the expression of the fetal alcohol syndrome .
	manualset3
210156	2	418291	7	NULL	NULL	0	NULL	degree of abnormality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The variation in the degree of abnormality found in dizygotic twins exposed to similar amounts of alcohol at the same time during gestation indicates that differences in fetal susceptibility to ethanol dysmorphogenesis are of prime importance to the expression of the fetal alcohol syndrome .
	manualset3
210157	3	418291	7	NULL	NULL	0	NULL	dizygotic twins	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The variation in the degree of abnormality found in dizygotic twins exposed to similar amounts of alcohol at the same time during gestation indicates that differences in fetal susceptibility to ethanol dysmorphogenesis are of prime importance to the expression of the fetal alcohol syndrome .
	manualset3
210158	4	418291	7	NULL	NULL	0	NULL	amounts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The variation in the degree of abnormality found in dizygotic twins exposed to similar amounts of alcohol at the same time during gestation indicates that differences in fetal susceptibility to ethanol dysmorphogenesis are of prime importance to the expression of the fetal alcohol syndrome .
	manualset3
210159	5	418291	7	NULL	NULL	0	NULL	alcohol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The variation in the degree of abnormality found in dizygotic twins exposed to similar amounts of alcohol at the same time during gestation indicates that differences in fetal susceptibility to ethanol dysmorphogenesis are of prime importance to the expression of the fetal alcohol syndrome .
	manualset3
210160	6	418291	7	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The variation in the degree of abnormality found in dizygotic twins exposed to similar amounts of alcohol at the same time during gestation indicates that differences in fetal susceptibility to ethanol dysmorphogenesis are of prime importance to the expression of the fetal alcohol syndrome .
	manualset3
210161	7	418291	7	NULL	NULL	0	NULL	gestation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The variation in the degree of abnormality found in dizygotic twins exposed to similar amounts of alcohol at the same time during gestation indicates that differences in fetal susceptibility to ethanol dysmorphogenesis are of prime importance to the expression of the fetal alcohol syndrome .
	manualset3
210162	8	418291	7	NULL	NULL	0	NULL	fetal susceptibility 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The variation in the degree of abnormality found in dizygotic twins exposed to similar amounts of alcohol at the same time during gestation indicates that differences in fetal susceptibility to ethanol dysmorphogenesis are of prime importance to the expression of the fetal alcohol syndrome .
	manualset3
210163	9	418291	7	NULL	NULL	0	NULL	ethanol dysmorphogenesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The variation in the degree of abnormality found in dizygotic twins exposed to similar amounts of alcohol at the same time during gestation indicates that differences in fetal susceptibility to ethanol dysmorphogenesis are of prime importance to the expression of the fetal alcohol syndrome .
	manualset3
210164	10	418291	7	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The variation in the degree of abnormality found in dizygotic twins exposed to similar amounts of alcohol at the same time during gestation indicates that differences in fetal susceptibility to ethanol dysmorphogenesis are of prime importance to the expression of the fetal alcohol syndrome .
	manualset3
210165	11	418291	7	NULL	NULL	0	NULL	fetal alcohol syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The variation in the degree of abnormality found in dizygotic twins exposed to similar amounts of alcohol at the same time during gestation indicates that differences in fetal susceptibility to ethanol dysmorphogenesis are of prime importance to the expression of the fetal alcohol syndrome .
	manualset3
210166	1	418292	7	NULL	NULL	0	NULL	values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , the values of the mean MSD exponent and effective diffusion coefficients can be traced back to negative correlations of the motion 's increments .
	manualset3
210167	2	418292	7	NULL	NULL	0	NULL	mean MSD exponent	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , the values of the mean MSD exponent and effective diffusion coefficients can be traced back to negative correlations of the motion 's increments .
	manualset3
210168	3	418292	7	NULL	NULL	0	NULL	 effective diffusion coefficients	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , the values of the mean MSD exponent and effective diffusion coefficients can be traced back to negative correlations of the motion 's increments .
	manualset3
210169	4	418292	7	NULL	NULL	0	NULL	negative correlations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , the values of the mean MSD exponent and effective diffusion coefficients can be traced back to negative correlations of the motion 's increments .
	manualset3
210170	5	418292	7	NULL	NULL	0	NULL	motion 's increments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , the values of the mean MSD exponent and effective diffusion coefficients can be traced back to negative correlations of the motion 's increments .
	manualset3
210171	1	418293	7	NULL	NULL	0	NULL	index calculations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The - index calculations can be finished within a few seconds for all 3D testing cases on one single NVIDIA Tesla C1060 card , achieving 45-75 speedup compared to CPU computations conducted on an Intel Xeon 2.27 GHz processor .
	manualset3
210172	2	418293	7	NULL	NULL	0	NULL	few seconds	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The - index calculations can be finished within a few seconds for all 3D testing cases on one single NVIDIA Tesla C1060 card , achieving 45-75 speedup compared to CPU computations conducted on an Intel Xeon 2.27 GHz processor .
	manualset3
210173	3	418293	7	NULL	NULL	NULL	NULL	3D testing cases	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The - index calculations can be finished within a few seconds for all 3D testing cases on one single NVIDIA Tesla C1060 card , achieving 45-75 speedup compared to CPU computations conducted on an Intel Xeon 2.27 GHz processor .
	manualset3
210174	4	418293	7	NULL	NULL	0	NULL	single NVIDIA Tesla C1060 card	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The - index calculations can be finished within a few seconds for all 3D testing cases on one single NVIDIA Tesla C1060 card , achieving 45-75 speedup compared to CPU computations conducted on an Intel Xeon 2.27 GHz processor .
	manualset3
210175	5	418293	7	NULL	NULL	0	NULL	45-75 speedup	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The - index calculations can be finished within a few seconds for all 3D testing cases on one single NVIDIA Tesla C1060 card , achieving 45-75 speedup compared to CPU computations conducted on an Intel Xeon 2.27 GHz processor .
	manualset3
210176	6	418293	7	NULL	NULL	0	NULL	CPU computations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The - index calculations can be finished within a few seconds for all 3D testing cases on one single NVIDIA Tesla C1060 card , achieving 45-75 speedup compared to CPU computations conducted on an Intel Xeon 2.27 GHz processor .
	manualset3
210177	7	418293	7	NULL	NULL	0	NULL	Intel Xeon 2.27 GHz processor	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The - index calculations can be finished within a few seconds for all 3D testing cases on one single NVIDIA Tesla C1060 card , achieving 45-75 speedup compared to CPU computations conducted on an Intel Xeon 2.27 GHz processor .
	manualset3
210228	1	418294	7	NULL	NULL	0	NULL	finding 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This finding is clinically relevant since TBX1 is the candidate for DGS/VCFS , characterized clinically by variable expressivity and reduced penetrance of cardiovascular defects ; Fgf8 gene variants may provide molecular clues to this variability .
	manualset3
210229	2	418294	7	NULL	NULL	0	NULL	TBX1	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	This finding is clinically relevant since TBX1 is the candidate for DGS/VCFS , characterized clinically by variable expressivity and reduced penetrance of cardiovascular defects ; Fgf8 gene variants may provide molecular clues to this variability .
	manualset3
210230	3	418294	7	NULL	NULL	0	NULL	DGS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This finding is clinically relevant since TBX1 is the candidate for DGS/VCFS , characterized clinically by variable expressivity and reduced penetrance of cardiovascular defects ; Fgf8 gene variants may provide molecular clues to this variability .
	manualset3
210231	4	418294	7	NULL	NULL	0	NULL	VCFS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This finding is clinically relevant since TBX1 is the candidate for DGS/VCFS , characterized clinically by variable expressivity and reduced penetrance of cardiovascular defects ; Fgf8 gene variants may provide molecular clues to this variability .
	manualset3
210232	5	418294	7	NULL	NULL	0	NULL	variable expressivity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This finding is clinically relevant since TBX1 is the candidate for DGS/VCFS , characterized clinically by variable expressivity and reduced penetrance of cardiovascular defects ; Fgf8 gene variants may provide molecular clues to this variability .
	manualset3
210233	6	418294	7	NULL	NULL	0	NULL	reduced penetrance	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This finding is clinically relevant since TBX1 is the candidate for DGS/VCFS , characterized clinically by variable expressivity and reduced penetrance of cardiovascular defects ; Fgf8 gene variants may provide molecular clues to this variability .
	manualset3
210234	7	418294	7	NULL	NULL	0	NULL	cardiovascular defects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This finding is clinically relevant since TBX1 is the candidate for DGS/VCFS , characterized clinically by variable expressivity and reduced penetrance of cardiovascular defects ; Fgf8 gene variants may provide molecular clues to this variability .
	manualset3
210235	8	418294	7	NULL	NULL	NULL	NULL	Fgf8 gene variants	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This finding is clinically relevant since TBX1 is the candidate for DGS/VCFS , characterized clinically by variable expressivity and reduced penetrance of cardiovascular defects ; Fgf8 gene variants may provide molecular clues to this variability .
	manualset3
210236	9	418294	7	NULL	NULL	0	NULL	 molecular clues 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This finding is clinically relevant since TBX1 is the candidate for DGS/VCFS , characterized clinically by variable expressivity and reduced penetrance of cardiovascular defects ; Fgf8 gene variants may provide molecular clues to this variability .
	manualset3
210237	10	418294	7	NULL	NULL	0	NULL	variability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This finding is clinically relevant since TBX1 is the candidate for DGS/VCFS , characterized clinically by variable expressivity and reduced penetrance of cardiovascular defects ; Fgf8 gene variants may provide molecular clues to this variability .
	manualset3
210238	1	418295	7	NULL	NULL	0	NULL	Clinical investigation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical investigation on globulin subfractions in serum and urine of patients with nephrotic syndrome .
	manualset3
210239	2	418295	7	NULL	NULL	0	NULL	globulin subfractions	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical investigation on globulin subfractions in serum and urine of patients with nephrotic syndrome .
	manualset3
210240	3	418295	7	NULL	NULL	0	NULL	 serum 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical investigation on globulin subfractions in serum and urine of patients with nephrotic syndrome .
	manualset3
210241	4	418295	7	NULL	NULL	0	NULL	urine 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical investigation on globulin subfractions in serum and urine of patients with nephrotic syndrome .
	manualset3
210242	5	418295	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical investigation on globulin subfractions in serum and urine of patients with nephrotic syndrome .
	manualset3
210243	6	418295	7	NULL	NULL	0	NULL	nephrotic syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical investigation on globulin subfractions in serum and urine of patients with nephrotic syndrome .
	manualset3
210244	1	418296	7	NULL	NULL	0	NULL	substitutions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Are substitutions in the first hypervariable region of the mitochondrial DNA displacement-loop in sudden infant death syndrome due to maternal inheritance ?
	manualset3
210245	2	418296	7	NULL	NULL	NULL	NULL	first hypervariable region	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Are substitutions in the first hypervariable region of the mitochondrial DNA displacement-loop in sudden infant death syndrome due to maternal inheritance ?
	manualset3
210246	3	418296	7	NULL	NULL	0	NULL	mitochondrial DNA displacement-loop	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Are substitutions in the first hypervariable region of the mitochondrial DNA displacement-loop in sudden infant death syndrome due to maternal inheritance ?
	manualset3
210247	4	418296	7	NULL	NULL	0	NULL	sudden infant death syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Are substitutions in the first hypervariable region of the mitochondrial DNA displacement-loop in sudden infant death syndrome due to maternal inheritance ?
	manualset3
210248	5	418296	7	NULL	NULL	0	NULL	maternal inheritance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Are substitutions in the first hypervariable region of the mitochondrial DNA displacement-loop in sudden infant death syndrome due to maternal inheritance ?
	manualset3
210249	1	418297	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of these studies are negative , equivocal , or , when positive , invalidated by methodologic defects or by inconsistency with the feasible carcinogenic effect of background radiation .
	manualset3
210250	2	418297	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of these studies are negative , equivocal , or , when positive , invalidated by methodologic defects or by inconsistency with the feasible carcinogenic effect of background radiation .
	manualset3
210251	3	418297	7	NULL	NULL	0	NULL	methodologic defects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of these studies are negative , equivocal , or , when positive , invalidated by methodologic defects or by inconsistency with the feasible carcinogenic effect of background radiation .
	manualset3
210252	4	418297	7	NULL	NULL	0	NULL	feasible carcinogenic effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of these studies are negative , equivocal , or , when positive , invalidated by methodologic defects or by inconsistency with the feasible carcinogenic effect of background radiation .
	manualset3
210253	5	418297	7	NULL	NULL	0	NULL	 background radiation 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of these studies are negative , equivocal , or , when positive , invalidated by methodologic defects or by inconsistency with the feasible carcinogenic effect of background radiation .
	manualset3
210258	1	418298	7	NULL	NULL	0	NULL	 strong correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The strong correlation between the number of nebulin modules and the length of skeletal muscle thin filaments in different species suggests that nebulin determines thin filament length .
	manualset3
210259	2	418298	7	NULL	NULL	0	NULL	 number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The strong correlation between the number of nebulin modules and the length of skeletal muscle thin filaments in different species suggests that nebulin determines thin filament length .
	manualset3
210260	3	418298	7	NULL	NULL	0	NULL	nebulin modules	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The strong correlation between the number of nebulin modules and the length of skeletal muscle thin filaments in different species suggests that nebulin determines thin filament length .
	manualset3
210261	4	418298	7	NULL	NULL	0	NULL	length	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The strong correlation between the number of nebulin modules and the length of skeletal muscle thin filaments in different species suggests that nebulin determines thin filament length .
	manualset3
210262	5	418298	7	NULL	NULL	0	NULL	skeletal muscle thin filaments	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The strong correlation between the number of nebulin modules and the length of skeletal muscle thin filaments in different species suggests that nebulin determines thin filament length .
	manualset3
210263	6	418298	7	NULL	NULL	0	NULL	species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The strong correlation between the number of nebulin modules and the length of skeletal muscle thin filaments in different species suggests that nebulin determines thin filament length .
	manualset3
210264	7	418298	7	NULL	NULL	0	NULL	nebulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The strong correlation between the number of nebulin modules and the length of skeletal muscle thin filaments in different species suggests that nebulin determines thin filament length .
	manualset3
210265	8	418298	7	NULL	NULL	0	NULL	thin filament length	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The strong correlation between the number of nebulin modules and the length of skeletal muscle thin filaments in different species suggests that nebulin determines thin filament length .
	manualset3
210442	1	418299	7	NULL	NULL	0	NULL	planetary isentrope	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Along the planetary isentrope water and ammonia behave as fully dissociated ionic , electronically insulating fluid phases , which turn metallic at temperatures exceeding 7000 kelvin for water and 5500 kelvin for ammonia .
	manualset3
210443	2	418299	7	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Along the planetary isentrope water and ammonia behave as fully dissociated ionic , electronically insulating fluid phases , which turn metallic at temperatures exceeding 7000 kelvin for water and 5500 kelvin for ammonia .
	manualset3
210444	3	418299	7	NULL	NULL	0	NULL	ammonia	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Along the planetary isentrope water and ammonia behave as fully dissociated ionic , electronically insulating fluid phases , which turn metallic at temperatures exceeding 7000 kelvin for water and 5500 kelvin for ammonia .
	manualset3
210445	4	418299	7	NULL	NULL	NULL	NULL	fully dissociated ionic , electronically insulating fluid phases	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Along the planetary isentrope water and ammonia behave as fully dissociated ionic , electronically insulating fluid phases , which turn metallic at temperatures exceeding 7000 kelvin for water and 5500 kelvin for ammonia .
	manualset3
210446	5	418299	7	NULL	NULL	0	NULL	temperatures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Along the planetary isentrope water and ammonia behave as fully dissociated ionic , electronically insulating fluid phases , which turn metallic at temperatures exceeding 7000 kelvin for water and 5500 kelvin for ammonia .
	manualset3
210447	6	418299	7	NULL	NULL	NULL	NULL	7000 kelvin	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Along the planetary isentrope water and ammonia behave as fully dissociated ionic , electronically insulating fluid phases , which turn metallic at temperatures exceeding 7000 kelvin for water and 5500 kelvin for ammonia .
	manualset3
210448	7	418299	7	NULL	NULL	0	NULL	 water 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Along the planetary isentrope water and ammonia behave as fully dissociated ionic , electronically insulating fluid phases , which turn metallic at temperatures exceeding 7000 kelvin for water and 5500 kelvin for ammonia .
	manualset3
210449	8	418299	7	NULL	NULL	0	NULL	5500 kelvin	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Along the planetary isentrope water and ammonia behave as fully dissociated ionic , electronically insulating fluid phases , which turn metallic at temperatures exceeding 7000 kelvin for water and 5500 kelvin for ammonia .
	manualset3
210450	9	418299	7	NULL	NULL	0	NULL	ammonia	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Along the planetary isentrope water and ammonia behave as fully dissociated ionic , electronically insulating fluid phases , which turn metallic at temperatures exceeding 7000 kelvin for water and 5500 kelvin for ammonia .
	manualset3
210451	1	418300	7	NULL	NULL	0	NULL	Secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Secretion of protein from salivary glands in the ferret in response to vasoactive intestinal peptide .
	manualset3
210452	2	418300	7	NULL	NULL	0	NULL	protein	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Secretion of protein from salivary glands in the ferret in response to vasoactive intestinal peptide .
	manualset3
210453	3	418300	7	NULL	NULL	0	NULL	salivary glands	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Secretion of protein from salivary glands in the ferret in response to vasoactive intestinal peptide .
	manualset3
210454	4	418300	7	NULL	NULL	0	NULL	ferret	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Secretion of protein from salivary glands in the ferret in response to vasoactive intestinal peptide .
	manualset3
210455	5	418300	7	NULL	NULL	0	NULL	vasoactive intestinal peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Secretion of protein from salivary glands in the ferret in response to vasoactive intestinal peptide .
	manualset3
210456	1	418301	7	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis that this observation is related to the simultaneous decreasing of a non-identified peak P3 or to the hydrolysis of a non-identified precursor as a quercetin heteroside is being investigated .
	manualset3
210457	2	418301	7	NULL	NULL	0	NULL	observation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis that this observation is related to the simultaneous decreasing of a non-identified peak P3 or to the hydrolysis of a non-identified precursor as a quercetin heteroside is being investigated .
	manualset3
210458	3	418301	7	NULL	NULL	0	NULL	 non-identified peak P3	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis that this observation is related to the simultaneous decreasing of a non-identified peak P3 or to the hydrolysis of a non-identified precursor as a quercetin heteroside is being investigated .
	manualset3
210459	4	418301	7	NULL	NULL	0	NULL	hydrolysis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis that this observation is related to the simultaneous decreasing of a non-identified peak P3 or to the hydrolysis of a non-identified precursor as a quercetin heteroside is being investigated .
	manualset3
210460	5	418301	7	NULL	NULL	0	NULL	non-identified precursor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis that this observation is related to the simultaneous decreasing of a non-identified peak P3 or to the hydrolysis of a non-identified precursor as a quercetin heteroside is being investigated .
	manualset3
210461	6	418301	7	NULL	NULL	0	NULL	quercetin heteroside	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis that this observation is related to the simultaneous decreasing of a non-identified peak P3 or to the hydrolysis of a non-identified precursor as a quercetin heteroside is being investigated .
	manualset3
210710	7	418301	7	NULL	NULL	0	NULL	decreasing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The hypothesis that this observation is related to the simultaneous decreasing of a non-identified peak P3 or to the hydrolysis of a non-identified precursor as a quercetin heteroside is being investigated .
	manualset3
210462	1	418302	7	NULL	NULL	0	NULL	 unique features	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These unique features may be more sensitive predictors of mortality than SDRR .
	manualset3
210463	2	418302	7	NULL	NULL	0	NULL	sensitive predictors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These unique features may be more sensitive predictors of mortality than SDRR .
	manualset3
210464	3	418302	7	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These unique features may be more sensitive predictors of mortality than SDRR .
	manualset3
210465	4	418302	7	NULL	NULL	0	NULL	SDRR 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These unique features may be more sensitive predictors of mortality than SDRR .
	manualset3
210466	1	418303	7	NULL	NULL	0	NULL	careful monitoring	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with careful monitoring of weight gain during pregnancy , early identification of a maladaptive response to the changes of pregnancy may help to avoid adverse outcomes .
	manualset3
210467	2	418303	7	NULL	NULL	0	NULL	weight gain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with careful monitoring of weight gain during pregnancy , early identification of a maladaptive response to the changes of pregnancy may help to avoid adverse outcomes .
	manualset3
210468	3	418303	7	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with careful monitoring of weight gain during pregnancy , early identification of a maladaptive response to the changes of pregnancy may help to avoid adverse outcomes .
	manualset3
210469	4	418303	7	NULL	NULL	0	NULL	early identification 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with careful monitoring of weight gain during pregnancy , early identification of a maladaptive response to the changes of pregnancy may help to avoid adverse outcomes .
	manualset3
210470	5	418303	7	NULL	NULL	0	NULL	maladaptive response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with careful monitoring of weight gain during pregnancy , early identification of a maladaptive response to the changes of pregnancy may help to avoid adverse outcomes .
	manualset3
210471	6	418303	7	NULL	NULL	0	NULL	changes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with careful monitoring of weight gain during pregnancy , early identification of a maladaptive response to the changes of pregnancy may help to avoid adverse outcomes .
	manualset3
210472	7	418303	7	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with careful monitoring of weight gain during pregnancy , early identification of a maladaptive response to the changes of pregnancy may help to avoid adverse outcomes .
	manualset3
210473	8	418303	7	NULL	NULL	0	NULL	adverse outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with careful monitoring of weight gain during pregnancy , early identification of a maladaptive response to the changes of pregnancy may help to avoid adverse outcomes .
	manualset3
210474	1	418304	7	NULL	NULL	0	NULL	Influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of hypovolemia on the pharmacokinetics and the electroencephalographic effect of propofol in the rat .
	manualset3
210475	2	418304	7	NULL	NULL	0	NULL	 hypovolemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of hypovolemia on the pharmacokinetics and the electroencephalographic effect of propofol in the rat .
	manualset3
210477	3	418304	7	NULL	NULL	0	NULL	pharmacokinetics effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of hypovolemia on the pharmacokinetics and the electroencephalographic effect of propofol in the rat .
	manualset3
210478	4	418304	7	NULL	NULL	0	NULL	electroencephalographic effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of hypovolemia on the pharmacokinetics and the electroencephalographic effect of propofol in the rat .
	manualset3
210479	5	418304	7	NULL	NULL	0	NULL	propofol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of hypovolemia on the pharmacokinetics and the electroencephalographic effect of propofol in the rat .
	manualset3
210480	6	418304	7	NULL	NULL	0	NULL	rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Influence of hypovolemia on the pharmacokinetics and the electroencephalographic effect of propofol in the rat .
	manualset3
210481	1	418305	7	NULL	NULL	0	NULL	Systemic candidiasis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Systemic candidiasis is the most frequently encountered opportunistic fungal infection , the kidneys being primarily affected in 80 % of the cases .
	manualset3
210482	2	418305	7	NULL	NULL	0	NULL	opportunistic fungal infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Systemic candidiasis is the most frequently encountered opportunistic fungal infection , the kidneys being primarily affected in 80 % of the cases .
	manualset3
210483	3	418305	7	NULL	NULL	0	NULL	kidneys	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Systemic candidiasis is the most frequently encountered opportunistic fungal infection , the kidneys being primarily affected in 80 % of the cases .
	manualset3
210484	4	418305	7	NULL	NULL	0	NULL	80 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Systemic candidiasis is the most frequently encountered opportunistic fungal infection , the kidneys being primarily affected in 80 % of the cases .
	manualset3
210485	5	418305	7	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Systemic candidiasis is the most frequently encountered opportunistic fungal infection , the kidneys being primarily affected in 80 % of the cases .
	manualset3
210486	1	418306	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , human endothelial cells were examined for susceptibility to EV71 infection using human microvascular endothelial cell line ( HMEC-1 cell ) .
	manualset3
210487	2	418306	7	NULL	NULL	0	NULL	human endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , human endothelial cells were examined for susceptibility to EV71 infection using human microvascular endothelial cell line ( HMEC-1 cell ) .
	manualset3
210488	3	418306	7	NULL	NULL	0	NULL	susceptibility 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , human endothelial cells were examined for susceptibility to EV71 infection using human microvascular endothelial cell line ( HMEC-1 cell ) .
	manualset3
210489	4	418306	7	NULL	NULL	0	NULL	EV71 infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , human endothelial cells were examined for susceptibility to EV71 infection using human microvascular endothelial cell line ( HMEC-1 cell ) .
	manualset3
210490	5	418306	7	NULL	NULL	0	NULL	human microvascular endothelial cell line ( HMEC-1 cell )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , human endothelial cells were examined for susceptibility to EV71 infection using human microvascular endothelial cell line ( HMEC-1 cell ) .
	manualset3
210491	1	418307	7	NULL	NULL	0	NULL	previous studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous studies , apoB polymorphisms have been shown to modify serum lipid responses to changes in dietary fat intake .
	manualset3
210492	2	418307	7	NULL	NULL	0	NULL	apoB polymorphisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous studies , apoB polymorphisms have been shown to modify serum lipid responses to changes in dietary fat intake .
	manualset3
210493	3	418307	7	NULL	NULL	0	NULL	serum lipid responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In previous studies , apoB polymorphisms have been shown to modify serum lipid responses to changes in dietary fat intake .
	manualset3
210494	4	418307	7	NULL	NULL	NULL	NULL	dietary fat intake	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In previous studies , apoB polymorphisms have been shown to modify serum lipid responses to changes in dietary fat intake .
	manualset3
210495	1	418308	7	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition we tested the hypothesis that these structural alterations in the dentate granule layer were associated with synaptic efficacy and thus muted long-term potentiation in mice lacking the protein .
	manualset3
210496	2	418308	7	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition we tested the hypothesis that these structural alterations in the dentate granule layer were associated with synaptic efficacy and thus muted long-term potentiation in mice lacking the protein .
	manualset3
210497	3	418308	7	NULL	NULL	0	NULL	structural alterations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition we tested the hypothesis that these structural alterations in the dentate granule layer were associated with synaptic efficacy and thus muted long-term potentiation in mice lacking the protein .
	manualset3
210498	4	418308	7	NULL	NULL	0	NULL	dentate granule layer 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition we tested the hypothesis that these structural alterations in the dentate granule layer were associated with synaptic efficacy and thus muted long-term potentiation in mice lacking the protein .
	manualset3
210499	5	418308	7	NULL	NULL	0	NULL	synaptic efficacy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition we tested the hypothesis that these structural alterations in the dentate granule layer were associated with synaptic efficacy and thus muted long-term potentiation in mice lacking the protein .
	manualset3
210500	6	418308	7	NULL	NULL	0	NULL	muted long-term potentiation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition we tested the hypothesis that these structural alterations in the dentate granule layer were associated with synaptic efficacy and thus muted long-term potentiation in mice lacking the protein .
	manualset3
210501	7	418308	7	NULL	NULL	0	NULL	 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition we tested the hypothesis that these structural alterations in the dentate granule layer were associated with synaptic efficacy and thus muted long-term potentiation in mice lacking the protein .
	manualset3
210502	8	418308	7	NULL	NULL	0	NULL	protein	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition we tested the hypothesis that these structural alterations in the dentate granule layer were associated with synaptic efficacy and thus muted long-term potentiation in mice lacking the protein .
	manualset3
210503	1	418309	7	NULL	NULL	0	NULL	examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An examination consisting of proton imaging , shimming and collection of 31P progressive saturation spectroscopic data for T1 determination required 1 h to perform .
	manualset3
210504	2	418309	7	NULL	NULL	0	NULL	proton imaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An examination consisting of proton imaging , shimming and collection of 31P progressive saturation spectroscopic data for T1 determination required 1 h to perform .
	manualset3
210505	3	418309	7	NULL	NULL	0	NULL	shimming	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An examination consisting of proton imaging , shimming and collection of 31P progressive saturation spectroscopic data for T1 determination required 1 h to perform .
	manualset3
210506	4	418309	7	NULL	NULL	0	NULL	collection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An examination consisting of proton imaging , shimming and collection of 31P progressive saturation spectroscopic data for T1 determination required 1 h to perform .
	manualset3
210507	5	418309	7	NULL	NULL	0	NULL	31P progressive saturation spectroscopic data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	An examination consisting of proton imaging , shimming and collection of 31P progressive saturation spectroscopic data for T1 determination required 1 h to perform .
	manualset3
210508	6	418309	7	NULL	NULL	0	NULL	T1 determination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An examination consisting of proton imaging , shimming and collection of 31P progressive saturation spectroscopic data for T1 determination required 1 h to perform .
	manualset3
210509	7	418309	7	NULL	NULL	0	NULL	 1 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	An examination consisting of proton imaging , shimming and collection of 31P progressive saturation spectroscopic data for T1 determination required 1 h to perform .
	manualset3
210510	1	418310	7	NULL	NULL	0	NULL	Trimethoprim	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Trimethoprim and enterococci in urinary tract infections : new perspectives on an old issue .
	manualset3
210511	2	418310	7	NULL	NULL	0	NULL	enterococci	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Trimethoprim and enterococci in urinary tract infections : new perspectives on an old issue .
	manualset3
210512	3	418310	7	NULL	NULL	0	NULL	urinary tract infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Trimethoprim and enterococci in urinary tract infections : new perspectives on an old issue .
	manualset3
210513	4	418310	7	NULL	NULL	0	NULL	new perspectives	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Trimethoprim and enterococci in urinary tract infections : new perspectives on an old issue .
	manualset3
210514	5	418310	7	NULL	NULL	0	NULL	old issue	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Trimethoprim and enterococci in urinary tract infections : new perspectives on an old issue .
	manualset3
210515	1	418311	7	NULL	NULL	0	NULL	noninvasive measurements	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with noninvasive measurements of electromyography ( EMG ) signals from respiratory muscles near the skin surface , it provides predictions for the forces generated by inner respiratory muscles as well as the instantaneous work of each muscle .
	manualset3
210516	2	418311	7	NULL	NULL	0	NULL	electromyography ( EMG ) signals 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with noninvasive measurements of electromyography ( EMG ) signals from respiratory muscles near the skin surface , it provides predictions for the forces generated by inner respiratory muscles as well as the instantaneous work of each muscle .
	manualset3
210517	3	418311	7	NULL	NULL	0	NULL	 respiratory muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with noninvasive measurements of electromyography ( EMG ) signals from respiratory muscles near the skin surface , it provides predictions for the forces generated by inner respiratory muscles as well as the instantaneous work of each muscle .
	manualset3
210518	4	418311	7	NULL	NULL	0	NULL	 skin surface	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with noninvasive measurements of electromyography ( EMG ) signals from respiratory muscles near the skin surface , it provides predictions for the forces generated by inner respiratory muscles as well as the instantaneous work of each muscle .
	manualset3
210519	5	418311	7	NULL	NULL	0	NULL	predictions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with noninvasive measurements of electromyography ( EMG ) signals from respiratory muscles near the skin surface , it provides predictions for the forces generated by inner respiratory muscles as well as the instantaneous work of each muscle .
	manualset3
210520	6	418311	7	NULL	NULL	0	NULL	forces	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with noninvasive measurements of electromyography ( EMG ) signals from respiratory muscles near the skin surface , it provides predictions for the forces generated by inner respiratory muscles as well as the instantaneous work of each muscle .
	manualset3
210521	7	418311	7	NULL	NULL	0	NULL	inner respiratory muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with noninvasive measurements of electromyography ( EMG ) signals from respiratory muscles near the skin surface , it provides predictions for the forces generated by inner respiratory muscles as well as the instantaneous work of each muscle .
	manualset3
210522	8	418311	7	NULL	NULL	0	NULL	instantaneous work	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with noninvasive measurements of electromyography ( EMG ) signals from respiratory muscles near the skin surface , it provides predictions for the forces generated by inner respiratory muscles as well as the instantaneous work of each muscle .
	manualset3
210523	9	418311	7	NULL	NULL	0	NULL	 muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with noninvasive measurements of electromyography ( EMG ) signals from respiratory muscles near the skin surface , it provides predictions for the forces generated by inner respiratory muscles as well as the instantaneous work of each muscle .
	manualset3
210524	1	418312	7	NULL	NULL	0	NULL	ends of hand-sealed gas-filled ampoules	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We have studied recently the ends of hand-sealed and machine-sealed , gas-filled ampoules of borosilicate glass .
	manualset3
210525	2	418312	7	NULL	NULL	0	NULL	machine-sealed gas-filled ampoules	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We have studied recently the ends of hand-sealed and machine-sealed , gas-filled ampoules of borosilicate glass .
	manualset3
210526	3	418312	7	NULL	NULL	0	NULL	borosilicate glass	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We have studied recently the ends of hand-sealed and machine-sealed , gas-filled ampoules of borosilicate glass .
	manualset3
210527	1	418313	7	NULL	NULL	0	NULL	evaluation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation showed that elbow dislocation without joint fracture has a favorable prognosis with return to complete functions .
	manualset3
210528	2	418313	7	NULL	NULL	0	NULL	elbow dislocation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation showed that elbow dislocation without joint fracture has a favorable prognosis with return to complete functions .
	manualset3
210529	3	418313	7	NULL	NULL	0	NULL	joint fracture	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation showed that elbow dislocation without joint fracture has a favorable prognosis with return to complete functions .
	manualset3
210530	4	418313	7	NULL	NULL	0	NULL	prognosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation showed that elbow dislocation without joint fracture has a favorable prognosis with return to complete functions .
	manualset3
210531	5	418313	7	NULL	NULL	0	NULL	 complete functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation showed that elbow dislocation without joint fracture has a favorable prognosis with return to complete functions .
	manualset3
210532	1	418314	7	NULL	NULL	0	NULL	Tissue engineering 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Tissue engineering of small diameter vascular grafts .
	manualset3
210533	2	418314	7	NULL	NULL	0	NULL	 small diameter vascular grafts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Tissue engineering of small diameter vascular grafts .
	manualset3
210534	1	418315	7	NULL	NULL	0	NULL	Genetic studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic studies have also renewed interest in previously studied pathways in IBD , such as the formation and function of the inflammasome and its relationship to interleukin ( IL ) 1-beta signaling .
	manualset3
210535	2	418315	7	NULL	NULL	0	NULL	 pathways	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic studies have also renewed interest in previously studied pathways in IBD , such as the formation and function of the inflammasome and its relationship to interleukin ( IL ) 1-beta signaling .
	manualset3
210536	3	418315	7	NULL	NULL	0	NULL	 IBD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic studies have also renewed interest in previously studied pathways in IBD , such as the formation and function of the inflammasome and its relationship to interleukin ( IL ) 1-beta signaling .
	manualset3
210537	4	418315	7	NULL	NULL	0	NULL	formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic studies have also renewed interest in previously studied pathways in IBD , such as the formation and function of the inflammasome and its relationship to interleukin ( IL ) 1-beta signaling .
	manualset3
210538	5	418315	7	NULL	NULL	0	NULL	 function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic studies have also renewed interest in previously studied pathways in IBD , such as the formation and function of the inflammasome and its relationship to interleukin ( IL ) 1-beta signaling .
	manualset3
210539	6	418315	7	NULL	NULL	0	NULL	 inflammasome	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic studies have also renewed interest in previously studied pathways in IBD , such as the formation and function of the inflammasome and its relationship to interleukin ( IL ) 1-beta signaling .
	manualset3
210540	7	418315	7	NULL	NULL	0	NULL	 relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic studies have also renewed interest in previously studied pathways in IBD , such as the formation and function of the inflammasome and its relationship to interleukin ( IL ) 1-beta signaling .
	manualset3
210541	8	418315	7	NULL	NULL	0	NULL	interleukin ( IL ) 1-beta signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic studies have also renewed interest in previously studied pathways in IBD , such as the formation and function of the inflammasome and its relationship to interleukin ( IL ) 1-beta signaling .
	manualset3
210542	1	418316	7	NULL	NULL	0	NULL	SP content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The SP content was not affected by age , sex or delay from death to freezing of tissue .
	manualset3
210543	2	418316	7	NULL	NULL	0	NULL	 age	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The SP content was not affected by age , sex or delay from death to freezing of tissue .
	manualset3
210544	3	418316	7	NULL	NULL	0	NULL	sex	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The SP content was not affected by age , sex or delay from death to freezing of tissue .
	manualset3
210545	4	418316	7	NULL	NULL	0	NULL	delay from death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The SP content was not affected by age , sex or delay from death to freezing of tissue .
	manualset3
210546	5	418316	7	NULL	NULL	0	NULL	freezing of tissue	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The SP content was not affected by age , sex or delay from death to freezing of tissue .
	manualset3
210547	1	418317	7	NULL	NULL	0	NULL	Infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants with abnormal lung function soon after birth may have a genetic predisposition to asthma or other airway abnormalities that predict the risk of subsequent lower respiratory tract illness .
	manualset3
210548	2	418317	7	NULL	NULL	0	NULL	abnormal lung function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants with abnormal lung function soon after birth may have a genetic predisposition to asthma or other airway abnormalities that predict the risk of subsequent lower respiratory tract illness .
	manualset3
210549	3	418317	7	NULL	NULL	0	NULL	birth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants with abnormal lung function soon after birth may have a genetic predisposition to asthma or other airway abnormalities that predict the risk of subsequent lower respiratory tract illness .
	manualset3
210550	4	418317	7	NULL	NULL	0	NULL	genetic predisposition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants with abnormal lung function soon after birth may have a genetic predisposition to asthma or other airway abnormalities that predict the risk of subsequent lower respiratory tract illness .
	manualset3
210551	5	418317	7	NULL	NULL	0	NULL	asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants with abnormal lung function soon after birth may have a genetic predisposition to asthma or other airway abnormalities that predict the risk of subsequent lower respiratory tract illness .
	manualset3
210552	6	418317	7	NULL	NULL	0	NULL	airway abnormalities	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants with abnormal lung function soon after birth may have a genetic predisposition to asthma or other airway abnormalities that predict the risk of subsequent lower respiratory tract illness .
	manualset3
210553	7	418317	7	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants with abnormal lung function soon after birth may have a genetic predisposition to asthma or other airway abnormalities that predict the risk of subsequent lower respiratory tract illness .
	manualset3
210554	8	418317	7	NULL	NULL	0	NULL	 lower respiratory tract illness 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infants with abnormal lung function soon after birth may have a genetic predisposition to asthma or other airway abnormalities that predict the risk of subsequent lower respiratory tract illness .
	manualset3
210555	1	418318	7	NULL	NULL	0	NULL	hydralazine SLE patient 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydralazine SLE patient had large amounts of autoantibodies that were predominantly IgG , while in the others IgM autoantibodies were predominant .
	manualset3
210556	2	418318	7	NULL	NULL	0	NULL	 large amounts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydralazine SLE patient had large amounts of autoantibodies that were predominantly IgG , while in the others IgM autoantibodies were predominant .
	manualset3
210557	3	418318	7	NULL	NULL	0	NULL	autoantibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydralazine SLE patient had large amounts of autoantibodies that were predominantly IgG , while in the others IgM autoantibodies were predominant .
	manualset3
210558	4	418318	7	NULL	NULL	0	NULL	 IgG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydralazine SLE patient had large amounts of autoantibodies that were predominantly IgG , while in the others IgM autoantibodies were predominant .
	manualset3
210559	5	418318	7	NULL	NULL	0	NULL	IgM autoantibodies	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The hydralazine SLE patient had large amounts of autoantibodies that were predominantly IgG , while in the others IgM autoantibodies were predominant .
	manualset3
210560	1	418319	7	NULL	NULL	0	NULL	fenaridine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with the above advantages fenaridine possesses all the complex of side effects typical of opiates associated with the depression of respiratory centres , psychoemotional sphere , activation of parasympathetic centres which may complicate the period following the patient 's withdrawal from anesthesia and necessitate prolonged controlled lung ventilation in the early postoperative period .
	manualset3
210561	2	418319	7	NULL	NULL	0	NULL	complex of side effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with the above advantages fenaridine possesses all the complex of side effects typical of opiates associated with the depression of respiratory centres , psychoemotional sphere , activation of parasympathetic centres which may complicate the period following the patient 's withdrawal from anesthesia and necessitate prolonged controlled lung ventilation in the early postoperative period .
	manualset3
210562	3	418319	7	NULL	NULL	0	NULL	opiates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with the above advantages fenaridine possesses all the complex of side effects typical of opiates associated with the depression of respiratory centres , psychoemotional sphere , activation of parasympathetic centres which may complicate the period following the patient 's withdrawal from anesthesia and necessitate prolonged controlled lung ventilation in the early postoperative period .
	manualset3
210563	4	418319	7	NULL	NULL	0	NULL	depression	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with the above advantages fenaridine possesses all the complex of side effects typical of opiates associated with the depression of respiratory centres , psychoemotional sphere , activation of parasympathetic centres which may complicate the period following the patient 's withdrawal from anesthesia and necessitate prolonged controlled lung ventilation in the early postoperative period .
	manualset3
210564	5	418319	7	NULL	NULL	0	NULL	respiratory centres	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with the above advantages fenaridine possesses all the complex of side effects typical of opiates associated with the depression of respiratory centres , psychoemotional sphere , activation of parasympathetic centres which may complicate the period following the patient 's withdrawal from anesthesia and necessitate prolonged controlled lung ventilation in the early postoperative period .
	manualset3
210565	6	418319	7	NULL	NULL	0	NULL	psychoemotional sphere	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with the above advantages fenaridine possesses all the complex of side effects typical of opiates associated with the depression of respiratory centres , psychoemotional sphere , activation of parasympathetic centres which may complicate the period following the patient 's withdrawal from anesthesia and necessitate prolonged controlled lung ventilation in the early postoperative period .
	manualset3
210566	7	418319	7	NULL	NULL	0	NULL	activation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with the above advantages fenaridine possesses all the complex of side effects typical of opiates associated with the depression of respiratory centres , psychoemotional sphere , activation of parasympathetic centres which may complicate the period following the patient 's withdrawal from anesthesia and necessitate prolonged controlled lung ventilation in the early postoperative period .
	manualset3
210567	8	418319	7	NULL	NULL	0	NULL	parasympathetic centres 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with the above advantages fenaridine possesses all the complex of side effects typical of opiates associated with the depression of respiratory centres , psychoemotional sphere , activation of parasympathetic centres which may complicate the period following the patient 's withdrawal from anesthesia and necessitate prolonged controlled lung ventilation in the early postoperative period .
	manualset3
210568	9	418319	7	NULL	NULL	0	NULL	period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with the above advantages fenaridine possesses all the complex of side effects typical of opiates associated with the depression of respiratory centres , psychoemotional sphere , activation of parasympathetic centres which may complicate the period following the patient 's withdrawal from anesthesia and necessitate prolonged controlled lung ventilation in the early postoperative period .
	manualset3
210569	10	418319	7	NULL	NULL	0	NULL	 patient 's withdrawal	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with the above advantages fenaridine possesses all the complex of side effects typical of opiates associated with the depression of respiratory centres , psychoemotional sphere , activation of parasympathetic centres which may complicate the period following the patient 's withdrawal from anesthesia and necessitate prolonged controlled lung ventilation in the early postoperative period .
	manualset3
210570	11	418319	7	NULL	NULL	0	NULL	anesthesia	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with the above advantages fenaridine possesses all the complex of side effects typical of opiates associated with the depression of respiratory centres , psychoemotional sphere , activation of parasympathetic centres which may complicate the period following the patient 's withdrawal from anesthesia and necessitate prolonged controlled lung ventilation in the early postoperative period .
	manualset3
210571	12	418319	7	NULL	NULL	0	NULL	controlled lung ventilation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with the above advantages fenaridine possesses all the complex of side effects typical of opiates associated with the depression of respiratory centres , psychoemotional sphere , activation of parasympathetic centres which may complicate the period following the patient 's withdrawal from anesthesia and necessitate prolonged controlled lung ventilation in the early postoperative period .
	manualset3
210572	13	418319	7	NULL	NULL	NULL	NULL	early postoperative period	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Along with the above advantages fenaridine possesses all the complex of side effects typical of opiates associated with the depression of respiratory centres , psychoemotional sphere , activation of parasympathetic centres which may complicate the period following the patient 's withdrawal from anesthesia and necessitate prolonged controlled lung ventilation in the early postoperative period .
	manualset3
210573	1	418320	7	NULL	NULL	0	NULL	Partial activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial activation , however , may be the overall result due to the lack of CD40 ligand expression , which may regulate costimulatory activity in APC and , in turn , may contribute to limiting the production of IL-2 required for T cell expansion and survival .
	manualset3
210574	2	418320	7	NULL	NULL	0	NULL	result 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial activation , however , may be the overall result due to the lack of CD40 ligand expression , which may regulate costimulatory activity in APC and , in turn , may contribute to limiting the production of IL-2 required for T cell expansion and survival .
	manualset3
210575	3	418320	7	NULL	NULL	0	NULL	CD40 ligand expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial activation , however , may be the overall result due to the lack of CD40 ligand expression , which may regulate costimulatory activity in APC and , in turn , may contribute to limiting the production of IL-2 required for T cell expansion and survival .
	manualset3
210576	4	418320	7	NULL	NULL	0	NULL	costimulatory activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial activation , however , may be the overall result due to the lack of CD40 ligand expression , which may regulate costimulatory activity in APC and , in turn , may contribute to limiting the production of IL-2 required for T cell expansion and survival .
	manualset3
210577	5	418320	7	NULL	NULL	0	NULL	APC 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial activation , however , may be the overall result due to the lack of CD40 ligand expression , which may regulate costimulatory activity in APC and , in turn , may contribute to limiting the production of IL-2 required for T cell expansion and survival .
	manualset3
210578	6	418320	7	NULL	NULL	0	NULL	production 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial activation , however , may be the overall result due to the lack of CD40 ligand expression , which may regulate costimulatory activity in APC and , in turn , may contribute to limiting the production of IL-2 required for T cell expansion and survival .
	manualset3
210579	7	418320	7	NULL	NULL	0	NULL	IL-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial activation , however , may be the overall result due to the lack of CD40 ligand expression , which may regulate costimulatory activity in APC and , in turn , may contribute to limiting the production of IL-2 required for T cell expansion and survival .
	manualset3
210580	8	418320	7	NULL	NULL	0	NULL	T cell expansion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial activation , however , may be the overall result due to the lack of CD40 ligand expression , which may regulate costimulatory activity in APC and , in turn , may contribute to limiting the production of IL-2 required for T cell expansion and survival .
	manualset3
210581	9	418320	7	NULL	NULL	0	NULL	survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial activation , however , may be the overall result due to the lack of CD40 ligand expression , which may regulate costimulatory activity in APC and , in turn , may contribute to limiting the production of IL-2 required for T cell expansion and survival .
	manualset3
210582	1	418321	7	NULL	NULL	0	NULL	 regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We find that this regulation is a highly specialized process that requires uncapped RNA , the HCV internal ribosome entry site ( IRES ) and the 3 ' region of miR-122 .
	manualset3
210583	2	418321	7	NULL	NULL	0	NULL	specialized process	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We find that this regulation is a highly specialized process that requires uncapped RNA , the HCV internal ribosome entry site ( IRES ) and the 3 ' region of miR-122 .
	manualset3
210584	3	418321	7	NULL	NULL	0	NULL	uncapped RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	We find that this regulation is a highly specialized process that requires uncapped RNA , the HCV internal ribosome entry site ( IRES ) and the 3 ' region of miR-122 .
	manualset3
210585	4	418321	7	NULL	NULL	0	NULL	HCV internal ribosome entry site ( IRES )	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	We find that this regulation is a highly specialized process that requires uncapped RNA , the HCV internal ribosome entry site ( IRES ) and the 3 ' region of miR-122 .
	manualset3
210586	5	418321	7	NULL	NULL	0	NULL	 3 ' region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	We find that this regulation is a highly specialized process that requires uncapped RNA , the HCV internal ribosome entry site ( IRES ) and the 3 ' region of miR-122 .
	manualset3
210587	6	418321	7	NULL	NULL	0	NULL	 miR-122	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	We find that this regulation is a highly specialized process that requires uncapped RNA , the HCV internal ribosome entry site ( IRES ) and the 3 ' region of miR-122 .
	manualset3
210588	1	418322	7	NULL	NULL	0	NULL	 whole-cell patch-clamp technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , using the whole-cell and single-channel patch-clamp technique , we investigated the effect of lidocaine , a local anesthetic , on the human ( h ) TREK1 channel heterologously expressed in human embryonic kidney 293 cells by an adenoviral-mediated expression system .
	manualset3
210589	2	418322	7	NULL	NULL	0	NULL	single-channel patch-clamp technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , using the whole-cell and single-channel patch-clamp technique , we investigated the effect of lidocaine , a local anesthetic , on the human ( h ) TREK1 channel heterologously expressed in human embryonic kidney 293 cells by an adenoviral-mediated expression system .
	manualset3
210590	3	418322	7	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , using the whole-cell and single-channel patch-clamp technique , we investigated the effect of lidocaine , a local anesthetic , on the human ( h ) TREK1 channel heterologously expressed in human embryonic kidney 293 cells by an adenoviral-mediated expression system .
	manualset3
210591	4	418322	7	NULL	NULL	0	NULL	lidocaine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , using the whole-cell and single-channel patch-clamp technique , we investigated the effect of lidocaine , a local anesthetic , on the human ( h ) TREK1 channel heterologously expressed in human embryonic kidney 293 cells by an adenoviral-mediated expression system .
	manualset3
210592	5	418322	7	NULL	NULL	0	NULL	local anesthetic	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , using the whole-cell and single-channel patch-clamp technique , we investigated the effect of lidocaine , a local anesthetic , on the human ( h ) TREK1 channel heterologously expressed in human embryonic kidney 293 cells by an adenoviral-mediated expression system .
	manualset3
210593	6	418322	7	NULL	NULL	0	NULL	human ( h ) TREK1 channel 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , using the whole-cell and single-channel patch-clamp technique , we investigated the effect of lidocaine , a local anesthetic , on the human ( h ) TREK1 channel heterologously expressed in human embryonic kidney 293 cells by an adenoviral-mediated expression system .
	manualset3
210594	7	418322	7	NULL	NULL	0	NULL	human embryonic kidney 293 cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , using the whole-cell and single-channel patch-clamp technique , we investigated the effect of lidocaine , a local anesthetic , on the human ( h ) TREK1 channel heterologously expressed in human embryonic kidney 293 cells by an adenoviral-mediated expression system .
	manualset3
210595	8	418322	7	NULL	NULL	0	NULL	adenoviral-mediated expression system	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , using the whole-cell and single-channel patch-clamp technique , we investigated the effect of lidocaine , a local anesthetic , on the human ( h ) TREK1 channel heterologously expressed in human embryonic kidney 293 cells by an adenoviral-mediated expression system .
	manualset3
210596	1	418323	7	NULL	NULL	0	NULL	dynamic CT scan	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , dynamic CT scan with air distention of the stomach revealed local thickening of stomach wall in 118 of 120 ( 98.3 % ) of the tumors and correctly determined their sizes in 106 of 120 ( 89.9 % ) .
	manualset3
210597	2	418323	7	NULL	NULL	NULL	NULL	air distention 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On the contrary , dynamic CT scan with air distention of the stomach revealed local thickening of stomach wall in 118 of 120 ( 98.3 % ) of the tumors and correctly determined their sizes in 106 of 120 ( 89.9 % ) .
	manualset3
210598	3	418323	7	NULL	NULL	0	NULL	stomach	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , dynamic CT scan with air distention of the stomach revealed local thickening of stomach wall in 118 of 120 ( 98.3 % ) of the tumors and correctly determined their sizes in 106 of 120 ( 89.9 % ) .
	manualset3
210599	4	418323	7	NULL	NULL	0	NULL	local thickening	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , dynamic CT scan with air distention of the stomach revealed local thickening of stomach wall in 118 of 120 ( 98.3 % ) of the tumors and correctly determined their sizes in 106 of 120 ( 89.9 % ) .
	manualset3
210600	5	418323	7	NULL	NULL	0	NULL	stomach wall 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , dynamic CT scan with air distention of the stomach revealed local thickening of stomach wall in 118 of 120 ( 98.3 % ) of the tumors and correctly determined their sizes in 106 of 120 ( 89.9 % ) .
	manualset3
210601	6	418323	7	NULL	NULL	0	NULL	118	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , dynamic CT scan with air distention of the stomach revealed local thickening of stomach wall in 118 of 120 ( 98.3 % ) of the tumors and correctly determined their sizes in 106 of 120 ( 89.9 % ) .
	manualset3
210602	7	418323	7	NULL	NULL	0	NULL	120	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , dynamic CT scan with air distention of the stomach revealed local thickening of stomach wall in 118 of 120 ( 98.3 % ) of the tumors and correctly determined their sizes in 106 of 120 ( 89.9 % ) .
	manualset3
210603	8	418323	7	NULL	NULL	0	NULL	98.3 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , dynamic CT scan with air distention of the stomach revealed local thickening of stomach wall in 118 of 120 ( 98.3 % ) of the tumors and correctly determined their sizes in 106 of 120 ( 89.9 % ) .
	manualset3
210604	9	418323	7	NULL	NULL	0	NULL	 tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , dynamic CT scan with air distention of the stomach revealed local thickening of stomach wall in 118 of 120 ( 98.3 % ) of the tumors and correctly determined their sizes in 106 of 120 ( 89.9 % ) .
	manualset3
210605	10	418323	7	NULL	NULL	0	NULL	sizes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , dynamic CT scan with air distention of the stomach revealed local thickening of stomach wall in 118 of 120 ( 98.3 % ) of the tumors and correctly determined their sizes in 106 of 120 ( 89.9 % ) .
	manualset3
210606	11	418323	7	NULL	NULL	0	NULL	106	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , dynamic CT scan with air distention of the stomach revealed local thickening of stomach wall in 118 of 120 ( 98.3 % ) of the tumors and correctly determined their sizes in 106 of 120 ( 89.9 % ) .
	manualset3
210607	12	418323	7	NULL	NULL	0	NULL	120 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , dynamic CT scan with air distention of the stomach revealed local thickening of stomach wall in 118 of 120 ( 98.3 % ) of the tumors and correctly determined their sizes in 106 of 120 ( 89.9 % ) .
	manualset3
210608	13	418323	7	NULL	NULL	0	NULL	89.9 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the contrary , dynamic CT scan with air distention of the stomach revealed local thickening of stomach wall in 118 of 120 ( 98.3 % ) of the tumors and correctly determined their sizes in 106 of 120 ( 89.9 % ) .
	manualset3
210609	1	418324	7	NULL	NULL	0	NULL	Reversibility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversibility of impaired renal function after long-term cyclosporin for psoriasis .
	manualset3
210610	2	418324	7	NULL	NULL	0	NULL	impaired renal function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversibility of impaired renal function after long-term cyclosporin for psoriasis .
	manualset3
210611	3	418324	7	NULL	NULL	NULL	NULL	long-term cyclosporin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Reversibility of impaired renal function after long-term cyclosporin for psoriasis .
	manualset3
210612	4	418324	7	NULL	NULL	0	NULL	 psoriasis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Reversibility of impaired renal function after long-term cyclosporin for psoriasis .
	manualset3
210613	1	418325	7	NULL	NULL	0	NULL	crystal	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal , inter-molecular N-HN hydrogen bonds connect the mol-ecules into a zigzag chain propagating in ( 100 ) .
	manualset3
210614	2	418325	7	NULL	NULL	0	NULL	inter-molecular N-HN hydrogen bonds	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal , inter-molecular N-HN hydrogen bonds connect the mol-ecules into a zigzag chain propagating in ( 100 ) .
	manualset3
210615	3	418325	7	NULL	NULL	0	NULL	 mol-ecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal , inter-molecular N-HN hydrogen bonds connect the mol-ecules into a zigzag chain propagating in ( 100 ) .
	manualset3
210616	4	418325	7	NULL	NULL	0	NULL	 zigzag chain	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal , inter-molecular N-HN hydrogen bonds connect the mol-ecules into a zigzag chain propagating in ( 100 ) .
	manualset3
210617	5	418325	7	NULL	NULL	0	NULL	100	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal , inter-molecular N-HN hydrogen bonds connect the mol-ecules into a zigzag chain propagating in ( 100 ) .
	manualset3
210618	1	418326	7	NULL	NULL	0	NULL	error	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports an error in `` Peer Influence on Risk Taking , Risk Preference , and Risky Decision Making in Adolescence and Adulthood : An Experimental Study '' by Margo Gardner and Laurence Steinberg ( Developmental Psychology , 2005 ( Jul ) , Vol 41 ( 4 ) , 625-635 ) .
	manualset3
210619	2	418326	7	NULL	NULL	0	NULL	` Peer Influence on Risk Taking , Risk Preference , and Risky Decision Making in Adolescence and Adulthood : An Experimental Study ''	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports an error in `` Peer Influence on Risk Taking , Risk Preference , and Risky Decision Making in Adolescence and Adulthood : An Experimental Study '' by Margo Gardner and Laurence Steinberg ( Developmental Psychology , 2005 ( Jul ) , Vol 41 ( 4 ) , 625-635 ) .
	manualset3
210621	3	418326	7	NULL	NULL	0	NULL	Margo Gardner	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports an error in `` Peer Influence on Risk Taking , Risk Preference , and Risky Decision Making in Adolescence and Adulthood : An Experimental Study '' by Margo Gardner and Laurence Steinberg ( Developmental Psychology , 2005 ( Jul ) , Vol 41 ( 4 ) , 625-635 ) .
	manualset3
210622	4	418326	7	NULL	NULL	0	NULL	Laurence Steinberg	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports an error in `` Peer Influence on Risk Taking , Risk Preference , and Risky Decision Making in Adolescence and Adulthood : An Experimental Study '' by Margo Gardner and Laurence Steinberg ( Developmental Psychology , 2005 ( Jul ) , Vol 41 ( 4 ) , 625-635 ) .
	manualset3
210623	5	418326	7	NULL	NULL	0	NULL	( Developmental Psychology , 2005 ( Jul ) , Vol 41 ( 4 ) , 625-635 )	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	Reports an error in `` Peer Influence on Risk Taking , Risk Preference , and Risky Decision Making in Adolescence and Adulthood : An Experimental Study '' by Margo Gardner and Laurence Steinberg ( Developmental Psychology , 2005 ( Jul ) , Vol 41 ( 4 ) , 625-635 ) .
	manualset3
210624	1	418327	7	NULL	NULL	0	NULL	Alpha-9 nicotinic acetylcholine receptor immunoreactivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Alpha-9 nicotinic acetylcholine receptor immunoreactivity in the rodent vestibular labyrinth .
	manualset3
210625	2	418327	7	NULL	NULL	0	NULL	rodent vestibular labyrinth	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Alpha-9 nicotinic acetylcholine receptor immunoreactivity in the rodent vestibular labyrinth .
	manualset3
210626	1	418328	7	NULL	NULL	0	NULL	Clinical analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical analysis shows that there are many distinct forms with or without nerve deafness , and with early or late occurrence of end-stage renal disease .
	manualset3
210627	2	418328	7	NULL	NULL	0	NULL	forms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical analysis shows that there are many distinct forms with or without nerve deafness , and with early or late occurrence of end-stage renal disease .
	manualset3
210628	3	418328	7	NULL	NULL	0	NULL	nerve deafness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical analysis shows that there are many distinct forms with or without nerve deafness , and with early or late occurrence of end-stage renal disease .
	manualset3
210629	4	418328	7	NULL	NULL	0	NULL	 early occurence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical analysis shows that there are many distinct forms with or without nerve deafness , and with early or late occurrence of end-stage renal disease .
	manualset3
210630	5	418328	7	NULL	NULL	0	NULL	 late occurrence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical analysis shows that there are many distinct forms with or without nerve deafness , and with early or late occurrence of end-stage renal disease .
	manualset3
210631	6	418328	7	NULL	NULL	0	NULL	end-stage renal disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical analysis shows that there are many distinct forms with or without nerve deafness , and with early or late occurrence of end-stage renal disease .
	manualset3
210632	1	418329	7	NULL	NULL	0	NULL	IVIG-nonresponders	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	IVIG-nonresponders had severe skin and muscle disease , concomitant with autoantibodies and/or malignancy .
	manualset3
210633	2	418329	7	NULL	NULL	0	NULL	skin disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	IVIG-nonresponders had severe skin and muscle disease , concomitant with autoantibodies and/or malignancy .
	manualset3
210634	3	418329	7	NULL	NULL	0	NULL	muscle disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	IVIG-nonresponders had severe skin and muscle disease , concomitant with autoantibodies and/or malignancy .
	manualset3
210635	4	418329	7	NULL	NULL	0	NULL	autoantibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	IVIG-nonresponders had severe skin and muscle disease , concomitant with autoantibodies and/or malignancy .
	manualset3
210636	5	418329	7	NULL	NULL	0	NULL	malignancy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	IVIG-nonresponders had severe skin and muscle disease , concomitant with autoantibodies and/or malignancy .
	manualset3
210637	1	418330	7	NULL	NULL	0	NULL	drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	For each drug , the minimal effective dose ( MED ) ( in milligrams per kilogram ) was defined as the lowest dose able to achieve a significant difference ( P less than 0.05 ) of CFU in the vegetations in comparison with controls 24 h after a single intravenous injection .
	manualset3
210638	2	418330	7	NULL	NULL	0	NULL	minimal effective dose ( MED ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For each drug , the minimal effective dose ( MED ) ( in milligrams per kilogram ) was defined as the lowest dose able to achieve a significant difference ( P less than 0.05 ) of CFU in the vegetations in comparison with controls 24 h after a single intravenous injection .
	manualset3
210639	3	418330	7	NULL	NULL	0	NULL	milligrams per kilogram	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For each drug , the minimal effective dose ( MED ) ( in milligrams per kilogram ) was defined as the lowest dose able to achieve a significant difference ( P less than 0.05 ) of CFU in the vegetations in comparison with controls 24 h after a single intravenous injection .
	manualset3
210640	4	418330	7	NULL	NULL	0	NULL	lowest dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For each drug , the minimal effective dose ( MED ) ( in milligrams per kilogram ) was defined as the lowest dose able to achieve a significant difference ( P less than 0.05 ) of CFU in the vegetations in comparison with controls 24 h after a single intravenous injection .
	manualset3
210641	5	418330	7	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	For each drug , the minimal effective dose ( MED ) ( in milligrams per kilogram ) was defined as the lowest dose able to achieve a significant difference ( P less than 0.05 ) of CFU in the vegetations in comparison with controls 24 h after a single intravenous injection .
	manualset3
210642	6	418330	7	NULL	NULL	0	NULL	P less than 0.05	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For each drug , the minimal effective dose ( MED ) ( in milligrams per kilogram ) was defined as the lowest dose able to achieve a significant difference ( P less than 0.05 ) of CFU in the vegetations in comparison with controls 24 h after a single intravenous injection .
	manualset3
210643	7	418330	7	NULL	NULL	0	NULL	CFU	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For each drug , the minimal effective dose ( MED ) ( in milligrams per kilogram ) was defined as the lowest dose able to achieve a significant difference ( P less than 0.05 ) of CFU in the vegetations in comparison with controls 24 h after a single intravenous injection .
	manualset3
210644	8	418330	7	NULL	NULL	NULL	NULL	vegetations	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For each drug , the minimal effective dose ( MED ) ( in milligrams per kilogram ) was defined as the lowest dose able to achieve a significant difference ( P less than 0.05 ) of CFU in the vegetations in comparison with controls 24 h after a single intravenous injection .
	manualset3
210645	9	418330	7	NULL	NULL	0	NULL	comparison	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For each drug , the minimal effective dose ( MED ) ( in milligrams per kilogram ) was defined as the lowest dose able to achieve a significant difference ( P less than 0.05 ) of CFU in the vegetations in comparison with controls 24 h after a single intravenous injection .
	manualset3
210646	10	418330	7	NULL	NULL	0	NULL	controls 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For each drug , the minimal effective dose ( MED ) ( in milligrams per kilogram ) was defined as the lowest dose able to achieve a significant difference ( P less than 0.05 ) of CFU in the vegetations in comparison with controls 24 h after a single intravenous injection .
	manualset3
210647	11	418330	7	NULL	NULL	0	NULL	24 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	For each drug , the minimal effective dose ( MED ) ( in milligrams per kilogram ) was defined as the lowest dose able to achieve a significant difference ( P less than 0.05 ) of CFU in the vegetations in comparison with controls 24 h after a single intravenous injection .
	manualset3
210648	12	418330	7	NULL	NULL	0	NULL	single intravenous injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For each drug , the minimal effective dose ( MED ) ( in milligrams per kilogram ) was defined as the lowest dose able to achieve a significant difference ( P less than 0.05 ) of CFU in the vegetations in comparison with controls 24 h after a single intravenous injection .
	manualset3
210728	1	419331	7	NULL	NULL	0	NULL	Vbl	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Vbl and pHi were measured with Ling-Gerard and liquid-membrane pH microelectrodes , respectively , in isolated tubules perfused in vitro .
	manualset3
210729	2	419331	7	NULL	NULL	0	NULL	pHi 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Vbl and pHi were measured with Ling-Gerard and liquid-membrane pH microelectrodes , respectively , in isolated tubules perfused in vitro .
	manualset3
210730	3	419331	7	NULL	NULL	0	NULL	Ling-Gerard	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Vbl and pHi were measured with Ling-Gerard and liquid-membrane pH microelectrodes , respectively , in isolated tubules perfused in vitro .
	manualset3
210731	4	419331	7	NULL	NULL	0	NULL	 liquid-membrane pH microelectrodes	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Vbl and pHi were measured with Ling-Gerard and liquid-membrane pH microelectrodes , respectively , in isolated tubules perfused in vitro .
	manualset3
210732	5	419331	7	NULL	NULL	0	NULL	isolated tubules	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Vbl and pHi were measured with Ling-Gerard and liquid-membrane pH microelectrodes , respectively , in isolated tubules perfused in vitro .
	manualset3
210759	1	419332	7	NULL	NULL	0	NULL	serological tests 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The serological tests ( liquid-phase ELISA and virus neutralization ) were able to distinguish between the three reference vaccine strains examined , but the five Indian field isolates reacted poorly with antisera produced against these vaccine strains .
	manualset3
210760	2	419332	7	NULL	NULL	0	NULL	 liquid-phase ELISA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The serological tests ( liquid-phase ELISA and virus neutralization ) were able to distinguish between the three reference vaccine strains examined , but the five Indian field isolates reacted poorly with antisera produced against these vaccine strains .
	manualset3
210761	3	419332	7	NULL	NULL	0	NULL	 virus neutralization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The serological tests ( liquid-phase ELISA and virus neutralization ) were able to distinguish between the three reference vaccine strains examined , but the five Indian field isolates reacted poorly with antisera produced against these vaccine strains .
	manualset3
210762	4	419332	7	NULL	NULL	NULL	NULL	three reference vaccine strains	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The serological tests ( liquid-phase ELISA and virus neutralization ) were able to distinguish between the three reference vaccine strains examined , but the five Indian field isolates reacted poorly with antisera produced against these vaccine strains .
	manualset3
210763	5	419332	7	NULL	NULL	0	NULL	five Indian field isolates	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The serological tests ( liquid-phase ELISA and virus neutralization ) were able to distinguish between the three reference vaccine strains examined , but the five Indian field isolates reacted poorly with antisera produced against these vaccine strains .
	manualset3
210765	6	419332	7	NULL	NULL	0	NULL	antisera	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The serological tests ( liquid-phase ELISA and virus neutralization ) were able to distinguish between the three reference vaccine strains examined , but the five Indian field isolates reacted poorly with antisera produced against these vaccine strains .
	manualset3
210767	7	419332	7	NULL	NULL	0	NULL	vaccine strains	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The serological tests ( liquid-phase ELISA and virus neutralization ) were able to distinguish between the three reference vaccine strains examined , but the five Indian field isolates reacted poorly with antisera produced against these vaccine strains .
	manualset3
210770	1	419333	7	NULL	NULL	0	NULL	bacterial sulfate reduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it has been demonstrated that bacterial sulfate reduction can be a key electron accepting process in many petroleum plumes , little is known about the rate of this reduction process in plumes derived from crude oil and gas condensates at cold-climate sites ( mean temperature & lt ; 10 degrees C ) , and in complex hydrogeological settings such as silt/clay aquitards .
	manualset3
210772	2	419333	7	NULL	NULL	0	NULL	electron accepting process	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it has been demonstrated that bacterial sulfate reduction can be a key electron accepting process in many petroleum plumes , little is known about the rate of this reduction process in plumes derived from crude oil and gas condensates at cold-climate sites ( mean temperature & lt ; 10 degrees C ) , and in complex hydrogeological settings such as silt/clay aquitards .
	manualset3
210775	3	419333	7	NULL	NULL	NULL	NULL	petroleum plumes	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although it has been demonstrated that bacterial sulfate reduction can be a key electron accepting process in many petroleum plumes , little is known about the rate of this reduction process in plumes derived from crude oil and gas condensates at cold-climate sites ( mean temperature & lt ; 10 degrees C ) , and in complex hydrogeological settings such as silt/clay aquitards .
	manualset3
210776	4	419333	7	NULL	NULL	0	NULL	 rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it has been demonstrated that bacterial sulfate reduction can be a key electron accepting process in many petroleum plumes , little is known about the rate of this reduction process in plumes derived from crude oil and gas condensates at cold-climate sites ( mean temperature & lt ; 10 degrees C ) , and in complex hydrogeological settings such as silt/clay aquitards .
	manualset3
210779	5	419333	7	NULL	NULL	0	NULL	reduction process	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it has been demonstrated that bacterial sulfate reduction can be a key electron accepting process in many petroleum plumes , little is known about the rate of this reduction process in plumes derived from crude oil and gas condensates at cold-climate sites ( mean temperature & lt ; 10 degrees C ) , and in complex hydrogeological settings such as silt/clay aquitards .
	manualset3
210783	6	419333	7	NULL	NULL	0	NULL	plumes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it has been demonstrated that bacterial sulfate reduction can be a key electron accepting process in many petroleum plumes , little is known about the rate of this reduction process in plumes derived from crude oil and gas condensates at cold-climate sites ( mean temperature & lt ; 10 degrees C ) , and in complex hydrogeological settings such as silt/clay aquitards .
	manualset3
210784	7	419333	7	NULL	NULL	0	NULL	 crude oil	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it has been demonstrated that bacterial sulfate reduction can be a key electron accepting process in many petroleum plumes , little is known about the rate of this reduction process in plumes derived from crude oil and gas condensates at cold-climate sites ( mean temperature & lt ; 10 degrees C ) , and in complex hydrogeological settings such as silt/clay aquitards .
	manualset3
210785	8	419333	7	NULL	NULL	0	NULL	gas 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it has been demonstrated that bacterial sulfate reduction can be a key electron accepting process in many petroleum plumes , little is known about the rate of this reduction process in plumes derived from crude oil and gas condensates at cold-climate sites ( mean temperature & lt ; 10 degrees C ) , and in complex hydrogeological settings such as silt/clay aquitards .
	manualset3
210786	9	419333	7	NULL	NULL	0	NULL	cold-climate sites	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it has been demonstrated that bacterial sulfate reduction can be a key electron accepting process in many petroleum plumes , little is known about the rate of this reduction process in plumes derived from crude oil and gas condensates at cold-climate sites ( mean temperature & lt ; 10 degrees C ) , and in complex hydrogeological settings such as silt/clay aquitards .
	manualset3
210788	10	419333	7	NULL	NULL	0	NULL	 mean temperature	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it has been demonstrated that bacterial sulfate reduction can be a key electron accepting process in many petroleum plumes , little is known about the rate of this reduction process in plumes derived from crude oil and gas condensates at cold-climate sites ( mean temperature & lt ; 10 degrees C ) , and in complex hydrogeological settings such as silt/clay aquitards .
	manualset3
210790	11	419333	7	NULL	NULL	0	NULL	& lt	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it has been demonstrated that bacterial sulfate reduction can be a key electron accepting process in many petroleum plumes , little is known about the rate of this reduction process in plumes derived from crude oil and gas condensates at cold-climate sites ( mean temperature & lt ; 10 degrees C ) , and in complex hydrogeological settings such as silt/clay aquitards .
	manualset3
210793	12	419333	7	NULL	NULL	0	NULL	10 degrees C	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it has been demonstrated that bacterial sulfate reduction can be a key electron accepting process in many petroleum plumes , little is known about the rate of this reduction process in plumes derived from crude oil and gas condensates at cold-climate sites ( mean temperature & lt ; 10 degrees C ) , and in complex hydrogeological settings such as silt/clay aquitards .
	manualset3
210796	13	419333	7	NULL	NULL	0	NULL	hydrogeological settings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it has been demonstrated that bacterial sulfate reduction can be a key electron accepting process in many petroleum plumes , little is known about the rate of this reduction process in plumes derived from crude oil and gas condensates at cold-climate sites ( mean temperature & lt ; 10 degrees C ) , and in complex hydrogeological settings such as silt/clay aquitards .
	manualset3
210798	14	419333	7	NULL	NULL	0	NULL	silt/clay aquitards	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it has been demonstrated that bacterial sulfate reduction can be a key electron accepting process in many petroleum plumes , little is known about the rate of this reduction process in plumes derived from crude oil and gas condensates at cold-climate sites ( mean temperature & lt ; 10 degrees C ) , and in complex hydrogeological settings such as silt/clay aquitards .
	manualset3
210809	1	419334	7	NULL	NULL	0	NULL	Control	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of salt gland activity in the hatchling green sea turtle , Chelonia mydas .
	manualset3
210810	2	419334	7	NULL	NULL	0	NULL	 salt gland activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of salt gland activity in the hatchling green sea turtle , Chelonia mydas .
	manualset3
210813	3	419334	7	NULL	NULL	0	NULL	 hatchling	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of salt gland activity in the hatchling green sea turtle , Chelonia mydas .
	manualset3
210814	4	419334	7	NULL	NULL	0	NULL	green sea turtle	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of salt gland activity in the hatchling green sea turtle , Chelonia mydas .
	manualset3
210815	5	419334	7	NULL	NULL	0	NULL	Chelonia mydas	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of salt gland activity in the hatchling green sea turtle , Chelonia mydas .
	manualset3
210816	1	419335	7	NULL	NULL	0	NULL	 human polymorphonuclear leukocyte ( PMN ) proteases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We determined whether human polymorphonuclear leukocyte ( PMN ) proteases contribute to asbestos-induced damage to human pulmonary epithelial-like cells ( PECs ) assessed using an in vitro chromium-51 release assay .
	manualset3
210817	2	419335	7	NULL	NULL	0	NULL	asbestos-induced damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We determined whether human polymorphonuclear leukocyte ( PMN ) proteases contribute to asbestos-induced damage to human pulmonary epithelial-like cells ( PECs ) assessed using an in vitro chromium-51 release assay .
	manualset3
210818	3	419335	7	NULL	NULL	0	NULL	 human pulmonary epithelial-like cells ( PECs )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We determined whether human polymorphonuclear leukocyte ( PMN ) proteases contribute to asbestos-induced damage to human pulmonary epithelial-like cells ( PECs ) assessed using an in vitro chromium-51 release assay .
	manualset3
210819	4	419335	7	NULL	NULL	0	NULL	in vitro chromium-51 release assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We determined whether human polymorphonuclear leukocyte ( PMN ) proteases contribute to asbestos-induced damage to human pulmonary epithelial-like cells ( PECs ) assessed using an in vitro chromium-51 release assay .
	manualset3
210820	1	419336	7	NULL	NULL	0	NULL	magnesium-deficient patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A magnesium-deficient patient presenting with hypocalcemia and hyperphosphatemia .
	manualset3
210821	2	419336	7	NULL	NULL	NULL	NULL	hypocalcemia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A magnesium-deficient patient presenting with hypocalcemia and hyperphosphatemia .
	manualset3
210822	3	419336	7	NULL	NULL	0	NULL	hyperphosphatemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A magnesium-deficient patient presenting with hypocalcemia and hyperphosphatemia .
	manualset3
210823	1	419337	7	NULL	NULL	0	NULL	Uterine blood flow	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Uterine blood flow during pregnancy is controlled by two distinct phenomena : phasic contractility and tone .
	manualset3
210824	2	419337	7	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Uterine blood flow during pregnancy is controlled by two distinct phenomena : phasic contractility and tone .
	manualset3
210825	3	419337	7	NULL	NULL	0	NULL	two distinct phenomena	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Uterine blood flow during pregnancy is controlled by two distinct phenomena : phasic contractility and tone .
	manualset3
210826	4	419337	7	NULL	NULL	0	NULL	phasic contractility	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Uterine blood flow during pregnancy is controlled by two distinct phenomena : phasic contractility and tone .
	manualset3
210827	5	419337	7	NULL	NULL	NULL	NULL	tone	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Uterine blood flow during pregnancy is controlled by two distinct phenomena : phasic contractility and tone .
	manualset3
210828	1	419338	7	NULL	NULL	0	NULL	regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These regions were not , however , sufficient to mediate up-regulation by the known Prdx6 inducers in our system .
	manualset3
210829	2	419338	7	NULL	NULL	0	NULL	up-regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These regions were not , however , sufficient to mediate up-regulation by the known Prdx6 inducers in our system .
	manualset3
210830	3	419338	7	NULL	NULL	0	NULL	Prdx6 inducers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These regions were not , however , sufficient to mediate up-regulation by the known Prdx6 inducers in our system .
	manualset3
210831	4	419338	7	NULL	NULL	0	NULL	 system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These regions were not , however , sufficient to mediate up-regulation by the known Prdx6 inducers in our system .
	manualset3
210832	1	419339	7	NULL	NULL	0	NULL	New method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( New method of quick bacteriological diagnosis of diphtheria ) .
	manualset3
210833	2	419339	7	NULL	NULL	0	NULL	quick bacteriological diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( New method of quick bacteriological diagnosis of diphtheria ) .
	manualset3
210834	3	419339	7	NULL	NULL	0	NULL	diphtheria	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( New method of quick bacteriological diagnosis of diphtheria ) .
	manualset3
210835	1	419340	7	NULL	NULL	0	NULL	Pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnancy following in vitro fertilization and embryo transfer by microsurgical epididymal sperm aspiration from a patient with congenital absence of the vas deferens : a case report .
	manualset3
210836	2	419340	7	NULL	NULL	0	NULL	in vitro fertilization 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnancy following in vitro fertilization and embryo transfer by microsurgical epididymal sperm aspiration from a patient with congenital absence of the vas deferens : a case report .
	manualset3
210837	3	419340	7	NULL	NULL	0	NULL	embryo transfer	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnancy following in vitro fertilization and embryo transfer by microsurgical epididymal sperm aspiration from a patient with congenital absence of the vas deferens : a case report .
	manualset3
210838	4	419340	7	NULL	NULL	0	NULL	microsurgical epididymal sperm aspiration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnancy following in vitro fertilization and embryo transfer by microsurgical epididymal sperm aspiration from a patient with congenital absence of the vas deferens : a case report .
	manualset3
210839	5	419340	7	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnancy following in vitro fertilization and embryo transfer by microsurgical epididymal sperm aspiration from a patient with congenital absence of the vas deferens : a case report .
	manualset3
210840	6	419340	7	NULL	NULL	0	NULL	congenital absence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnancy following in vitro fertilization and embryo transfer by microsurgical epididymal sperm aspiration from a patient with congenital absence of the vas deferens : a case report .
	manualset3
210841	7	419340	7	NULL	NULL	0	NULL	vas deferens	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnancy following in vitro fertilization and embryo transfer by microsurgical epididymal sperm aspiration from a patient with congenital absence of the vas deferens : a case report .
	manualset3
210842	8	419340	7	NULL	NULL	0	NULL	case report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnancy following in vitro fertilization and embryo transfer by microsurgical epididymal sperm aspiration from a patient with congenital absence of the vas deferens : a case report .
	manualset3
210843	1	419341	7	NULL	NULL	0	NULL	Prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of oral lesions and smokeless tobacco use in Northern Plains Indians .
	manualset3
210844	2	419341	7	NULL	NULL	0	NULL	 oral lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of oral lesions and smokeless tobacco use in Northern Plains Indians .
	manualset3
210845	3	419341	7	NULL	NULL	0	NULL	smokeless tobacco use	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of oral lesions and smokeless tobacco use in Northern Plains Indians .
	manualset3
210846	4	419341	7	NULL	NULL	0	NULL	Northern Plains Indians 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of oral lesions and smokeless tobacco use in Northern Plains Indians .
	manualset3
210847	1	419342	7	NULL	NULL	0	NULL	Agonist-induced desensitization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Agonist-induced desensitization of adenosine A1 and A2 receptors was studied in rat striatum slices maintained in carbo-oxygenated Krebs buffer .
	manualset3
210848	2	419342	7	NULL	NULL	0	NULL	 adenosine A1 receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Agonist-induced desensitization of adenosine A1 and A2 receptors was studied in rat striatum slices maintained in carbo-oxygenated Krebs buffer .
	manualset3
210849	3	419342	7	NULL	NULL	0	NULL	A2 receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Agonist-induced desensitization of adenosine A1 and A2 receptors was studied in rat striatum slices maintained in carbo-oxygenated Krebs buffer .
	manualset3
210850	4	419342	7	NULL	NULL	0	NULL	rat striatum slices	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Agonist-induced desensitization of adenosine A1 and A2 receptors was studied in rat striatum slices maintained in carbo-oxygenated Krebs buffer .
	manualset3
210851	5	419342	7	NULL	NULL	0	NULL	carbo-oxygenated Krebs buffer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Agonist-induced desensitization of adenosine A1 and A2 receptors was studied in rat striatum slices maintained in carbo-oxygenated Krebs buffer .
	manualset3
210852	1	419343	7	NULL	NULL	0	NULL	voluntary questionnaire	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A voluntary questionnaire on leukapheresis was sent to 280 FDA-registered blood-collecting establishments performing leukapheresis .
	manualset3
210853	2	419343	7	NULL	NULL	NULL	NULL	 leukapheresis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A voluntary questionnaire on leukapheresis was sent to 280 FDA-registered blood-collecting establishments performing leukapheresis .
	manualset3
210854	3	419343	7	NULL	NULL	0	NULL	280 FDA-registered blood-collecting establishments 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A voluntary questionnaire on leukapheresis was sent to 280 FDA-registered blood-collecting establishments performing leukapheresis .
	manualset3
210855	4	419343	7	NULL	NULL	0	NULL	leukapheresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A voluntary questionnaire on leukapheresis was sent to 280 FDA-registered blood-collecting establishments performing leukapheresis .
	manualset3
210856	1	419344	7	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it has been recognized from the study of individual isolates that these associations are individually important for plant growth , little is known about interactions of whole assemblages of beneficial and pathogenic microorganisms associating with plants .
	manualset3
210857	2	419344	7	NULL	NULL	0	NULL	individual isolates	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it has been recognized from the study of individual isolates that these associations are individually important for plant growth , little is known about interactions of whole assemblages of beneficial and pathogenic microorganisms associating with plants .
	manualset3
210858	3	419344	7	NULL	NULL	0	NULL	associations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it has been recognized from the study of individual isolates that these associations are individually important for plant growth , little is known about interactions of whole assemblages of beneficial and pathogenic microorganisms associating with plants .
	manualset3
210859	4	419344	7	NULL	NULL	0	NULL	 plant growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it has been recognized from the study of individual isolates that these associations are individually important for plant growth , little is known about interactions of whole assemblages of beneficial and pathogenic microorganisms associating with plants .
	manualset3
210860	5	419344	7	NULL	NULL	0	NULL	 interactions	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it has been recognized from the study of individual isolates that these associations are individually important for plant growth , little is known about interactions of whole assemblages of beneficial and pathogenic microorganisms associating with plants .
	manualset3
210861	6	419344	7	NULL	NULL	0	NULL	whole assemblages 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it has been recognized from the study of individual isolates that these associations are individually important for plant growth , little is known about interactions of whole assemblages of beneficial and pathogenic microorganisms associating with plants .
	manualset3
210862	7	419344	7	NULL	NULL	0	NULL	beneficial microorganisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it has been recognized from the study of individual isolates that these associations are individually important for plant growth , little is known about interactions of whole assemblages of beneficial and pathogenic microorganisms associating with plants .
	manualset3
210863	8	419344	7	NULL	NULL	0	NULL	pathogenic microorganisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it has been recognized from the study of individual isolates that these associations are individually important for plant growth , little is known about interactions of whole assemblages of beneficial and pathogenic microorganisms associating with plants .
	manualset3
210864	9	419344	7	NULL	NULL	0	NULL	plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it has been recognized from the study of individual isolates that these associations are individually important for plant growth , little is known about interactions of whole assemblages of beneficial and pathogenic microorganisms associating with plants .
	manualset3
210865	1	419345	7	NULL	NULL	0	NULL	one surgical disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There is one surgical disease that provides considerable experience of the process of screening over a period of 30 years and this is congenital dislocation of the hip ( CDH ) .
	manualset3
210866	2	419345	7	NULL	NULL	0	NULL	experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is one surgical disease that provides considerable experience of the process of screening over a period of 30 years and this is congenital dislocation of the hip ( CDH ) .
	manualset3
210867	3	419345	7	NULL	NULL	0	NULL	process of screening 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is one surgical disease that provides considerable experience of the process of screening over a period of 30 years and this is congenital dislocation of the hip ( CDH ) .
	manualset3
210868	4	419345	7	NULL	NULL	0	NULL	 period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	There is one surgical disease that provides considerable experience of the process of screening over a period of 30 years and this is congenital dislocation of the hip ( CDH ) .
	manualset3
210869	5	419345	7	NULL	NULL	0	NULL	30 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	There is one surgical disease that provides considerable experience of the process of screening over a period of 30 years and this is congenital dislocation of the hip ( CDH ) .
	manualset3
210870	6	419345	7	NULL	NULL	0	NULL	 congenital dislocation of the hip ( CDH )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is one surgical disease that provides considerable experience of the process of screening over a period of 30 years and this is congenital dislocation of the hip ( CDH ) .
	manualset3
210871	1	419346	7	NULL	NULL	0	NULL	genetic predisposition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A genetic predisposition to form HO is suspected but not proven .
	manualset3
210872	2	419346	7	NULL	NULL	0	NULL	HO	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A genetic predisposition to form HO is suspected but not proven .
	manualset3
210873	1	419347	7	NULL	NULL	NULL	NULL	methamphetamine ( METH )	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The use of methamphetamine ( METH ) is a growing public health problem , because its abuse is associated with long-term biochemical and structural effects on the human brain .
	manualset3
210874	2	419347	7	NULL	NULL	0	NULL	public health problem	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of methamphetamine ( METH ) is a growing public health problem , because its abuse is associated with long-term biochemical and structural effects on the human brain .
	manualset3
210875	3	419347	7	NULL	NULL	0	NULL	abuse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of methamphetamine ( METH ) is a growing public health problem , because its abuse is associated with long-term biochemical and structural effects on the human brain .
	manualset3
210876	4	419347	7	NULL	NULL	0	NULL	 long-term biochemical effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of methamphetamine ( METH ) is a growing public health problem , because its abuse is associated with long-term biochemical and structural effects on the human brain .
	manualset3
210877	5	419347	7	NULL	NULL	0	NULL	structural effects 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of methamphetamine ( METH ) is a growing public health problem , because its abuse is associated with long-term biochemical and structural effects on the human brain .
	manualset3
210878	6	419347	7	NULL	NULL	0	NULL	human brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of methamphetamine ( METH ) is a growing public health problem , because its abuse is associated with long-term biochemical and structural effects on the human brain .
	manualset3
212847	7	419347	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of methamphetamine ( METH ) is a growing public health problem , because its abuse is associated with long-term biochemical and structural effects on the human brain .
	manualset3
210879	1	419348	7	NULL	NULL	0	NULL	Evaluation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluation of the accessory nerve and trapezius muscle was performed on eight subjects with neck dissection secondary to oropharyngeal/laryngeal cancer .
	manualset3
210880	2	419348	7	NULL	NULL	0	NULL	 accessory nerve	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluation of the accessory nerve and trapezius muscle was performed on eight subjects with neck dissection secondary to oropharyngeal/laryngeal cancer .
	manualset3
210881	3	419348	7	NULL	NULL	0	NULL	trapezius muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluation of the accessory nerve and trapezius muscle was performed on eight subjects with neck dissection secondary to oropharyngeal/laryngeal cancer .
	manualset3
210882	4	419348	7	NULL	NULL	0	NULL	eight subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluation of the accessory nerve and trapezius muscle was performed on eight subjects with neck dissection secondary to oropharyngeal/laryngeal cancer .
	manualset3
210883	5	419348	7	NULL	NULL	0	NULL	neck dissection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluation of the accessory nerve and trapezius muscle was performed on eight subjects with neck dissection secondary to oropharyngeal/laryngeal cancer .
	manualset3
210884	6	419348	7	NULL	NULL	0	NULL	oropharyngeal/laryngeal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluation of the accessory nerve and trapezius muscle was performed on eight subjects with neck dissection secondary to oropharyngeal/laryngeal cancer .
	manualset3
210885	1	419349	7	NULL	NULL	0	NULL	Manganese superoxide dismutase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Manganese superoxide dismutase was detected within some articular and epiphyseal chondrocytes , within some osteoprogenitor cells and osteoblasts , within many osteoclasts , and within some vascular smooth muscle cells .
	manualset3
210886	2	419349	7	NULL	NULL	0	NULL	articular chondrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Manganese superoxide dismutase was detected within some articular and epiphyseal chondrocytes , within some osteoprogenitor cells and osteoblasts , within many osteoclasts , and within some vascular smooth muscle cells .
	manualset3
210887	3	419349	7	NULL	NULL	0	NULL	epiphyseal chondrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Manganese superoxide dismutase was detected within some articular and epiphyseal chondrocytes , within some osteoprogenitor cells and osteoblasts , within many osteoclasts , and within some vascular smooth muscle cells .
	manualset3
210888	4	419349	7	NULL	NULL	0	NULL	osteoprogenitor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Manganese superoxide dismutase was detected within some articular and epiphyseal chondrocytes , within some osteoprogenitor cells and osteoblasts , within many osteoclasts , and within some vascular smooth muscle cells .
	manualset3
210889	5	419349	7	NULL	NULL	0	NULL	osteoblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Manganese superoxide dismutase was detected within some articular and epiphyseal chondrocytes , within some osteoprogenitor cells and osteoblasts , within many osteoclasts , and within some vascular smooth muscle cells .
	manualset3
210890	7	419349	7	NULL	NULL	NULL	NULL	vascular smooth muscle cells 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Manganese superoxide dismutase was detected within some articular and epiphyseal chondrocytes , within some osteoprogenitor cells and osteoblasts , within many osteoclasts , and within some vascular smooth muscle cells .
	manualset3
210891	6	419349	7	NULL	NULL	0	NULL	 osteoclasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Manganese superoxide dismutase was detected within some articular and epiphyseal chondrocytes , within some osteoprogenitor cells and osteoblasts , within many osteoclasts , and within some vascular smooth muscle cells .
	manualset3
210892	1	419350	7	NULL	NULL	NULL	NULL	auto -RNPs	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the latter case , both auto - and heterologous alpha RNPs were seen to penetrate , whereas only autologous alpha RNPs entered LRec-1 cells .
	manualset3
210893	2	419350	7	NULL	NULL	NULL	NULL	heterologous alpha RNPs	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the latter case , both auto - and heterologous alpha RNPs were seen to penetrate , whereas only autologous alpha RNPs entered LRec-1 cells .
	manualset3
210894	3	419350	7	NULL	NULL	0	NULL	autologous alpha RNPs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the latter case , both auto - and heterologous alpha RNPs were seen to penetrate , whereas only autologous alpha RNPs entered LRec-1 cells .
	manualset3
210895	4	419350	7	NULL	NULL	0	NULL	LRec-1 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the latter case , both auto - and heterologous alpha RNPs were seen to penetrate , whereas only autologous alpha RNPs entered LRec-1 cells .
	manualset3
210898	1	419351	7	NULL	NULL	0	NULL	Diffusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Diffusion of mycoheptin from the discs into agar was studied .
	manualset3
210900	2	419351	7	NULL	NULL	0	NULL	mycoheptin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Diffusion of mycoheptin from the discs into agar was studied .
	manualset3
210903	3	419351	7	NULL	NULL	0	NULL	discs	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Diffusion of mycoheptin from the discs into agar was studied .
	manualset3
210904	4	419351	7	NULL	NULL	0	NULL	agar	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Diffusion of mycoheptin from the discs into agar was studied .
	manualset3
210909	1	419352	7	NULL	NULL	0	NULL	chemokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it has been shown that chemokines bind and activate their respective G protein-coupled receptors as monomers , many chemokines oligomerize upon GAG binding , and the ability to oligomerize and bind GAGs is required for in vivo function .
	manualset3
210911	2	419352	7	NULL	NULL	0	NULL	G protein-coupled receptors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it has been shown that chemokines bind and activate their respective G protein-coupled receptors as monomers , many chemokines oligomerize upon GAG binding , and the ability to oligomerize and bind GAGs is required for in vivo function .
	manualset3
210912	3	419352	7	NULL	NULL	0	NULL	monomers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it has been shown that chemokines bind and activate their respective G protein-coupled receptors as monomers , many chemokines oligomerize upon GAG binding , and the ability to oligomerize and bind GAGs is required for in vivo function .
	manualset3
210914	4	419352	7	NULL	NULL	0	NULL	chemokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it has been shown that chemokines bind and activate their respective G protein-coupled receptors as monomers , many chemokines oligomerize upon GAG binding , and the ability to oligomerize and bind GAGs is required for in vivo function .
	manualset3
210916	5	419352	7	NULL	NULL	0	NULL	GAG binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it has been shown that chemokines bind and activate their respective G protein-coupled receptors as monomers , many chemokines oligomerize upon GAG binding , and the ability to oligomerize and bind GAGs is required for in vivo function .
	manualset3
210917	6	419352	7	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it has been shown that chemokines bind and activate their respective G protein-coupled receptors as monomers , many chemokines oligomerize upon GAG binding , and the ability to oligomerize and bind GAGs is required for in vivo function .
	manualset3
210919	7	419352	7	NULL	NULL	0	NULL	GAGs	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it has been shown that chemokines bind and activate their respective G protein-coupled receptors as monomers , many chemokines oligomerize upon GAG binding , and the ability to oligomerize and bind GAGs is required for in vivo function .
	manualset3
210921	8	419352	7	NULL	NULL	0	NULL	 in vivo function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it has been shown that chemokines bind and activate their respective G protein-coupled receptors as monomers , many chemokines oligomerize upon GAG binding , and the ability to oligomerize and bind GAGs is required for in vivo function .
	manualset3
210922	1	419353	7	NULL	NULL	0	NULL	 entropy changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The entropy and affinity changes that accompanied agonist binding suggested that agonists induced significant conformational changes in intact acetylcholine receptors .
	manualset3
210923	2	419353	7	NULL	NULL	0	NULL	affinity changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The entropy and affinity changes that accompanied agonist binding suggested that agonists induced significant conformational changes in intact acetylcholine receptors .
	manualset3
210924	3	419353	7	NULL	NULL	0	NULL	agonist binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The entropy and affinity changes that accompanied agonist binding suggested that agonists induced significant conformational changes in intact acetylcholine receptors .
	manualset3
210925	4	419353	7	NULL	NULL	0	NULL	agonists	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The entropy and affinity changes that accompanied agonist binding suggested that agonists induced significant conformational changes in intact acetylcholine receptors .
	manualset3
210926	5	419353	7	NULL	NULL	0	NULL	conformational changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The entropy and affinity changes that accompanied agonist binding suggested that agonists induced significant conformational changes in intact acetylcholine receptors .
	manualset3
210927	6	419353	7	NULL	NULL	0	NULL	acetylcholine receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The entropy and affinity changes that accompanied agonist binding suggested that agonists induced significant conformational changes in intact acetylcholine receptors .
	manualset3
210928	1	419354	7	NULL	NULL	0	NULL	 dose 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	At this dose , the activation of the shell of the nucleus accumbens occurred together with that of the core of the nucleus accumbens and of most other brain regions .
	manualset3
210929	2	419354	7	NULL	NULL	0	NULL	activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	At this dose , the activation of the shell of the nucleus accumbens occurred together with that of the core of the nucleus accumbens and of most other brain regions .
	manualset3
210930	3	419354	7	NULL	NULL	0	NULL	 shell of the nucleus accumbens	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	At this dose , the activation of the shell of the nucleus accumbens occurred together with that of the core of the nucleus accumbens and of most other brain regions .
	manualset3
210931	4	419354	7	NULL	NULL	0	NULL	 core of the nucleus accumbens	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	At this dose , the activation of the shell of the nucleus accumbens occurred together with that of the core of the nucleus accumbens and of most other brain regions .
	manualset3
210932	5	419354	7	NULL	NULL	0	NULL	 brain regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	At this dose , the activation of the shell of the nucleus accumbens occurred together with that of the core of the nucleus accumbens and of most other brain regions .
	manualset3
210933	1	419355	7	NULL	NULL	0	NULL	Energy savings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Energy savings of 67 % attributed to posture were calculated .
	manualset3
210934	2	419355	7	NULL	NULL	0	NULL	67 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Energy savings of 67 % attributed to posture were calculated .
	manualset3
210935	3	419355	7	NULL	NULL	0	NULL	 posture	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Energy savings of 67 % attributed to posture were calculated .
	manualset3
210936	1	419356	7	NULL	NULL	0	NULL	Homes	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Homes supplied with gas as main energy source had significantly higher concentrations of CO2 , CO and NO2 .
	manualset3
210937	2	419356	7	NULL	NULL	0	NULL	 gas	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Homes supplied with gas as main energy source had significantly higher concentrations of CO2 , CO and NO2 .
	manualset3
210938	3	419356	7	NULL	NULL	0	NULL	main energy source	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Homes supplied with gas as main energy source had significantly higher concentrations of CO2 , CO and NO2 .
	manualset3
210939	4	419356	7	NULL	NULL	0	NULL	higher concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Homes supplied with gas as main energy source had significantly higher concentrations of CO2 , CO and NO2 .
	manualset3
210940	5	419356	7	NULL	NULL	0	NULL	CO2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Homes supplied with gas as main energy source had significantly higher concentrations of CO2 , CO and NO2 .
	manualset3
210941	6	419356	7	NULL	NULL	0	NULL	CO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Homes supplied with gas as main energy source had significantly higher concentrations of CO2 , CO and NO2 .
	manualset3
210942	7	419356	7	NULL	NULL	0	NULL	NO2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Homes supplied with gas as main energy source had significantly higher concentrations of CO2 , CO and NO2 .
	manualset3
210944	1	419357	7	NULL	NULL	0	NULL	metabolites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolites of histamine , tele-methylhistamine ( t-MH ) and tele-methylimidazoleacetic acid ( t-MIAA ) , were measured in cerebrospinal fluid ( CSF ) from 47 subjects with neurological disorders and healthy controls .
	manualset3
210945	2	419357	7	NULL	NULL	0	NULL	histamine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolites of histamine , tele-methylhistamine ( t-MH ) and tele-methylimidazoleacetic acid ( t-MIAA ) , were measured in cerebrospinal fluid ( CSF ) from 47 subjects with neurological disorders and healthy controls .
	manualset3
210947	3	419357	7	NULL	NULL	0	NULL	tele-methylhistamine ( t-MH ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolites of histamine , tele-methylhistamine ( t-MH ) and tele-methylimidazoleacetic acid ( t-MIAA ) , were measured in cerebrospinal fluid ( CSF ) from 47 subjects with neurological disorders and healthy controls .
	manualset3
210948	4	419357	7	NULL	NULL	0	NULL	tele-methylimidazoleacetic acid ( t-MIAA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolites of histamine , tele-methylhistamine ( t-MH ) and tele-methylimidazoleacetic acid ( t-MIAA ) , were measured in cerebrospinal fluid ( CSF ) from 47 subjects with neurological disorders and healthy controls .
	manualset3
210949	5	419357	7	NULL	NULL	0	NULL	 cerebrospinal fluid ( CSF )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolites of histamine , tele-methylhistamine ( t-MH ) and tele-methylimidazoleacetic acid ( t-MIAA ) , were measured in cerebrospinal fluid ( CSF ) from 47 subjects with neurological disorders and healthy controls .
	manualset3
210950	6	419357	7	NULL	NULL	0	NULL	47 subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolites of histamine , tele-methylhistamine ( t-MH ) and tele-methylimidazoleacetic acid ( t-MIAA ) , were measured in cerebrospinal fluid ( CSF ) from 47 subjects with neurological disorders and healthy controls .
	manualset3
210951	7	419357	7	NULL	NULL	0	NULL	neurological disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolites of histamine , tele-methylhistamine ( t-MH ) and tele-methylimidazoleacetic acid ( t-MIAA ) , were measured in cerebrospinal fluid ( CSF ) from 47 subjects with neurological disorders and healthy controls .
	manualset3
210953	8	419357	7	NULL	NULL	0	NULL	 healthy controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The metabolites of histamine , tele-methylhistamine ( t-MH ) and tele-methylimidazoleacetic acid ( t-MIAA ) , were measured in cerebrospinal fluid ( CSF ) from 47 subjects with neurological disorders and healthy controls .
	manualset3
210954	1	419358	7	NULL	NULL	0	NULL	2 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 2 patients there was specific lymph node involvement .
	manualset3
210965	2	419358	7	NULL	NULL	0	NULL	lymph node	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In 2 patients there was specific lymph node involvement .
	manualset3
210967	1	419359	7	NULL	NULL	0	NULL	 respiratory rate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiratory rate is a vital sign that can provide important information about the health of a patient , especially that of the respiratory system .
	manualset3
210968	2	419359	7	NULL	NULL	0	NULL	vital sign	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiratory rate is a vital sign that can provide important information about the health of a patient , especially that of the respiratory system .
	manualset3
210970	3	419359	7	NULL	NULL	0	NULL	information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiratory rate is a vital sign that can provide important information about the health of a patient , especially that of the respiratory system .
	manualset3
210971	4	419359	7	NULL	NULL	0	NULL	health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiratory rate is a vital sign that can provide important information about the health of a patient , especially that of the respiratory system .
	manualset3
210972	5	419359	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiratory rate is a vital sign that can provide important information about the health of a patient , especially that of the respiratory system .
	manualset3
210973	6	419359	7	NULL	NULL	0	NULL	respiratory system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The respiratory rate is a vital sign that can provide important information about the health of a patient , especially that of the respiratory system .
	manualset3
210974	1	419360	7	NULL	NULL	0	NULL	IgA changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IgA and IgG changes were less consistent .
	manualset3
210975	2	419360	7	NULL	NULL	0	NULL	IgG changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IgA and IgG changes were less consistent .
	manualset3
211077	1	419361	7	NULL	NULL	0	NULL	Hypoxic radiosensitizers	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	( 2 ) Hypoxic radiosensitizers and bioreductive drugs .
	manualset3
211078	2	419361	7	NULL	NULL	0	NULL	bioreductive drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( 2 ) Hypoxic radiosensitizers and bioreductive drugs .
	manualset3
211079	1	419362	7	NULL	NULL	NULL	NULL	nuclear architecture	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although it is generally accepted that nuclear architecture is an important determinant of nuclear activity , it is not clear whether cytoplasmic events , such as transcript localization and cell polarity , are affected by this architecture .
	manualset3
211080	2	419362	7	NULL	NULL	0	NULL	nuclear activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it is generally accepted that nuclear architecture is an important determinant of nuclear activity , it is not clear whether cytoplasmic events , such as transcript localization and cell polarity , are affected by this architecture .
	manualset3
211081	3	419362	7	NULL	NULL	0	NULL	cytoplasmic events	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it is generally accepted that nuclear architecture is an important determinant of nuclear activity , it is not clear whether cytoplasmic events , such as transcript localization and cell polarity , are affected by this architecture .
	manualset3
211082	4	419362	7	NULL	NULL	0	NULL	transcript localization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it is generally accepted that nuclear architecture is an important determinant of nuclear activity , it is not clear whether cytoplasmic events , such as transcript localization and cell polarity , are affected by this architecture .
	manualset3
211083	5	419362	7	NULL	NULL	0	NULL	cell polarity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it is generally accepted that nuclear architecture is an important determinant of nuclear activity , it is not clear whether cytoplasmic events , such as transcript localization and cell polarity , are affected by this architecture .
	manualset3
211084	6	419362	7	NULL	NULL	0	NULL	architecture	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although it is generally accepted that nuclear architecture is an important determinant of nuclear activity , it is not clear whether cytoplasmic events , such as transcript localization and cell polarity , are affected by this architecture .
	manualset3
211085	1	419363	7	NULL	NULL	NULL	NULL	 baseline examinations	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As baseline examinations , width of the keratinized gingiva , probing pocket depth , position of the gingival margin , and the clinical attachment level were recorded and oral photographs were taken .
	manualset3
211086	2	419363	7	NULL	NULL	0	NULL	width	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As baseline examinations , width of the keratinized gingiva , probing pocket depth , position of the gingival margin , and the clinical attachment level were recorded and oral photographs were taken .
	manualset3
211087	3	419363	7	NULL	NULL	NULL	NULL	keratinized gingiva	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As baseline examinations , width of the keratinized gingiva , probing pocket depth , position of the gingival margin , and the clinical attachment level were recorded and oral photographs were taken .
	manualset3
211088	4	419363	7	NULL	NULL	NULL	NULL	probing pocket depth	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As baseline examinations , width of the keratinized gingiva , probing pocket depth , position of the gingival margin , and the clinical attachment level were recorded and oral photographs were taken .
	manualset3
211089	5	419363	7	NULL	NULL	0	NULL	position	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As baseline examinations , width of the keratinized gingiva , probing pocket depth , position of the gingival margin , and the clinical attachment level were recorded and oral photographs were taken .
	manualset3
211090	6	419363	7	NULL	NULL	0	NULL	 gingival margin	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As baseline examinations , width of the keratinized gingiva , probing pocket depth , position of the gingival margin , and the clinical attachment level were recorded and oral photographs were taken .
	manualset3
211091	7	419363	7	NULL	NULL	0	NULL	clinical attachment level	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As baseline examinations , width of the keratinized gingiva , probing pocket depth , position of the gingival margin , and the clinical attachment level were recorded and oral photographs were taken .
	manualset3
211092	8	419363	7	NULL	NULL	NULL	NULL	oral photographs	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As baseline examinations , width of the keratinized gingiva , probing pocket depth , position of the gingival margin , and the clinical attachment level were recorded and oral photographs were taken .
	manualset3
211093	1	419364	7	NULL	NULL	NULL	NULL	regioisomers 3a	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The regioisomers 3a and 3b ; 4a and 4b were separated by column chromatography and characterized for evaluation of the antiplatelet effects in rabbit washed platelets and human platelet-rich plasma .
	manualset3
211094	2	419364	7	NULL	NULL	NULL	NULL	regioisomers 3b	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The regioisomers 3a and 3b ; 4a and 4b were separated by column chromatography and characterized for evaluation of the antiplatelet effects in rabbit washed platelets and human platelet-rich plasma .
	manualset3
211095	3	419364	7	NULL	NULL	NULL	NULL	regioisomers 4a	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The regioisomers 3a and 3b ; 4a and 4b were separated by column chromatography and characterized for evaluation of the antiplatelet effects in rabbit washed platelets and human platelet-rich plasma .
	manualset3
211096	4	419364	7	NULL	NULL	NULL	NULL	regioisomers 4b	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The regioisomers 3a and 3b ; 4a and 4b were separated by column chromatography and characterized for evaluation of the antiplatelet effects in rabbit washed platelets and human platelet-rich plasma .
	manualset3
211097	5	419364	7	NULL	NULL	0	NULL	column chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The regioisomers 3a and 3b ; 4a and 4b were separated by column chromatography and characterized for evaluation of the antiplatelet effects in rabbit washed platelets and human platelet-rich plasma .
	manualset3
211098	6	419364	7	NULL	NULL	0	NULL	evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The regioisomers 3a and 3b ; 4a and 4b were separated by column chromatography and characterized for evaluation of the antiplatelet effects in rabbit washed platelets and human platelet-rich plasma .
	manualset3
211099	7	419364	7	NULL	NULL	0	NULL	antiplatelet effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The regioisomers 3a and 3b ; 4a and 4b were separated by column chromatography and characterized for evaluation of the antiplatelet effects in rabbit washed platelets and human platelet-rich plasma .
	manualset3
211100	8	419364	7	NULL	NULL	0	NULL	rabbit washed platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The regioisomers 3a and 3b ; 4a and 4b were separated by column chromatography and characterized for evaluation of the antiplatelet effects in rabbit washed platelets and human platelet-rich plasma .
	manualset3
211101	9	419364	7	NULL	NULL	0	NULL	human platelet-rich plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The regioisomers 3a and 3b ; 4a and 4b were separated by column chromatography and characterized for evaluation of the antiplatelet effects in rabbit washed platelets and human platelet-rich plasma .
	manualset3
211102	1	419365	7	NULL	NULL	0	NULL	Pregnant rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnant rats were housed under normoxic ( 21 % O ( 2 ) ) or hypoxic ( 13 % O ( 2 ) ) conditions from day 6 to day 20 of gestation .
	manualset3
211103	2	419365	7	NULL	NULL	NULL	NULL	normoxic conditions	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pregnant rats were housed under normoxic ( 21 % O ( 2 ) ) or hypoxic ( 13 % O ( 2 ) ) conditions from day 6 to day 20 of gestation .
	manualset3
211104	3	419365	7	NULL	NULL	0	NULL	21 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnant rats were housed under normoxic ( 21 % O ( 2 ) ) or hypoxic ( 13 % O ( 2 ) ) conditions from day 6 to day 20 of gestation .
	manualset3
211105	4	419365	7	NULL	NULL	0	NULL	O ( 2 ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnant rats were housed under normoxic ( 21 % O ( 2 ) ) or hypoxic ( 13 % O ( 2 ) ) conditions from day 6 to day 20 of gestation .
	manualset3
211106	5	419365	7	NULL	NULL	NULL	NULL	hypoxic conditions	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pregnant rats were housed under normoxic ( 21 % O ( 2 ) ) or hypoxic ( 13 % O ( 2 ) ) conditions from day 6 to day 20 of gestation .
	manualset3
211107	6	419365	7	NULL	NULL	0	NULL	13 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnant rats were housed under normoxic ( 21 % O ( 2 ) ) or hypoxic ( 13 % O ( 2 ) ) conditions from day 6 to day 20 of gestation .
	manualset3
211108	7	419365	7	NULL	NULL	0	NULL	O ( 2 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnant rats were housed under normoxic ( 21 % O ( 2 ) ) or hypoxic ( 13 % O ( 2 ) ) conditions from day 6 to day 20 of gestation .
	manualset3
211109	8	419365	7	NULL	NULL	0	NULL	 day 6	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnant rats were housed under normoxic ( 21 % O ( 2 ) ) or hypoxic ( 13 % O ( 2 ) ) conditions from day 6 to day 20 of gestation .
	manualset3
211110	9	419365	7	NULL	NULL	0	NULL	day 20	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnant rats were housed under normoxic ( 21 % O ( 2 ) ) or hypoxic ( 13 % O ( 2 ) ) conditions from day 6 to day 20 of gestation .
	manualset3
211111	10	419365	7	NULL	NULL	0	NULL	gestation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnant rats were housed under normoxic ( 21 % O ( 2 ) ) or hypoxic ( 13 % O ( 2 ) ) conditions from day 6 to day 20 of gestation .
	manualset3
211112	1	419366	7	NULL	NULL	0	NULL	 analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These analyses reveal that predictions of future population fluctuations of weakly density-regulated populations such as the ibex often become uncertain .
	manualset3
211113	2	419366	7	NULL	NULL	0	NULL	predictions	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These analyses reveal that predictions of future population fluctuations of weakly density-regulated populations such as the ibex often become uncertain .
	manualset3
211114	3	419366	7	NULL	NULL	0	NULL	 future population fluctuations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These analyses reveal that predictions of future population fluctuations of weakly density-regulated populations such as the ibex often become uncertain .
	manualset3
211115	4	419366	7	NULL	NULL	0	NULL	weakly density-regulated populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These analyses reveal that predictions of future population fluctuations of weakly density-regulated populations such as the ibex often become uncertain .
	manualset3
211116	5	419366	7	NULL	NULL	0	NULL	 ibex	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These analyses reveal that predictions of future population fluctuations of weakly density-regulated populations such as the ibex often become uncertain .
	manualset3
211117	1	419367	7	NULL	NULL	0	NULL	Roentgenologic study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Roentgenologic study of solitary peripheral lung mass with emphasis on correlation to pulmonary vasculatures ) .
	manualset3
211118	2	419367	7	NULL	NULL	NULL	NULL	solitary peripheral lung mass 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Roentgenologic study of solitary peripheral lung mass with emphasis on correlation to pulmonary vasculatures ) .
	manualset3
211119	3	419367	7	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	( Roentgenologic study of solitary peripheral lung mass with emphasis on correlation to pulmonary vasculatures ) .
	manualset3
211120	4	419367	7	NULL	NULL	0	NULL	pulmonary vasculatures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Roentgenologic study of solitary peripheral lung mass with emphasis on correlation to pulmonary vasculatures ) .
	manualset3
211121	1	419368	7	NULL	NULL	NULL	NULL	 exponential state-growth languages	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Learning exponential state-growth languages by hill climbing .
	manualset3
211122	2	419368	7	NULL	NULL	0	NULL	hill climbing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Learning exponential state-growth languages by hill climbing .
	manualset3
212924	3	419368	7	NULL	NULL	0	NULL	Learning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Learning exponential state-growth languages by hill climbing .
	manualset3
211123	1	419369	7	NULL	NULL	0	NULL	Endogenous activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Endogenous activities of phospholipases A and C in Ureaplasma urealyticum were assayed in cellular fractions of exponential-phase cells .
	manualset3
211124	2	419369	7	NULL	NULL	0	NULL	phospholipases A 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Endogenous activities of phospholipases A and C in Ureaplasma urealyticum were assayed in cellular fractions of exponential-phase cells .
	manualset3
211125	3	419369	7	NULL	NULL	0	NULL	phospholipases C	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Endogenous activities of phospholipases A and C in Ureaplasma urealyticum were assayed in cellular fractions of exponential-phase cells .
	manualset3
211126	4	419369	7	NULL	NULL	0	NULL	Ureaplasma urealyticum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Endogenous activities of phospholipases A and C in Ureaplasma urealyticum were assayed in cellular fractions of exponential-phase cells .
	manualset3
211127	5	419369	7	NULL	NULL	0	NULL	cellular fractions	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Endogenous activities of phospholipases A and C in Ureaplasma urealyticum were assayed in cellular fractions of exponential-phase cells .
	manualset3
211128	6	419369	7	NULL	NULL	0	NULL	exponential-phase cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Endogenous activities of phospholipases A and C in Ureaplasma urealyticum were assayed in cellular fractions of exponential-phase cells .
	manualset3
211129	1	419370	7	NULL	NULL	0	NULL	kinetic parameters	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetic parameters for cathepsin G are significantly slower than those for many other serine proteases .
	manualset3
211130	2	419370	7	NULL	NULL	0	NULL	cathepsin G	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetic parameters for cathepsin G are significantly slower than those for many other serine proteases .
	manualset3
211131	3	419370	7	NULL	NULL	0	NULL	serine proteases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetic parameters for cathepsin G are significantly slower than those for many other serine proteases .
	manualset3
211132	1	419371	7	NULL	NULL	0	NULL	 discovery	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The discovery of ghrelin and its role in human metabolism has promoted significant research and advances in the study of obesity and other weight-related disorders .
	manualset3
211133	2	419371	7	NULL	NULL	0	NULL	 ghrelin	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The discovery of ghrelin and its role in human metabolism has promoted significant research and advances in the study of obesity and other weight-related disorders .
	manualset3
211134	3	419371	7	NULL	NULL	0	NULL	 role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The discovery of ghrelin and its role in human metabolism has promoted significant research and advances in the study of obesity and other weight-related disorders .
	manualset3
211135	4	419371	7	NULL	NULL	NULL	NULL	human metabolism 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The discovery of ghrelin and its role in human metabolism has promoted significant research and advances in the study of obesity and other weight-related disorders .
	manualset3
211136	5	419371	7	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The discovery of ghrelin and its role in human metabolism has promoted significant research and advances in the study of obesity and other weight-related disorders .
	manualset3
211137	6	419371	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The discovery of ghrelin and its role in human metabolism has promoted significant research and advances in the study of obesity and other weight-related disorders .
	manualset3
211138	7	419371	7	NULL	NULL	NULL	NULL	obesity	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The discovery of ghrelin and its role in human metabolism has promoted significant research and advances in the study of obesity and other weight-related disorders .
	manualset3
211139	8	419371	7	NULL	NULL	0	NULL	 weight-related disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The discovery of ghrelin and its role in human metabolism has promoted significant research and advances in the study of obesity and other weight-related disorders .
	manualset3
212933	9	419371	7	NULL	NULL	0	NULL	advances	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The discovery of ghrelin and its role in human metabolism has promoted significant research and advances in the study of obesity and other weight-related disorders .
	manualset3
211140	1	419372	7	NULL	NULL	0	NULL	Lysine levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysine levels increased and phenylalanine fell .
	manualset3
211141	2	419372	7	NULL	NULL	NULL	NULL	 phenylalanine	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Lysine levels increased and phenylalanine fell .
	manualset3
211162	1	419373	7	NULL	NULL	0	NULL	Initial experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial experience with the use of porcine acellular dermal matrix ( Strattice ) for abdominal wall reinforcement after transverse rectus abdominis myocutaneous flap breast reconstruction .
	manualset3
211163	2	419373	7	NULL	NULL	0	NULL	porcine acellular dermal matrix ( Strattice )	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial experience with the use of porcine acellular dermal matrix ( Strattice ) for abdominal wall reinforcement after transverse rectus abdominis myocutaneous flap breast reconstruction .
	manualset3
211164	3	419373	7	NULL	NULL	0	NULL	abdominal wall reinforcement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial experience with the use of porcine acellular dermal matrix ( Strattice ) for abdominal wall reinforcement after transverse rectus abdominis myocutaneous flap breast reconstruction .
	manualset3
211165	4	419373	7	NULL	NULL	0	NULL	transverse rectus abdominis myocutaneous flap breast reconstruction	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial experience with the use of porcine acellular dermal matrix ( Strattice ) for abdominal wall reinforcement after transverse rectus abdominis myocutaneous flap breast reconstruction .
	manualset3
211166	1	419374	7	NULL	NULL	0	NULL	THE FOUNDATION FOR INDUSTRIAL RESEARCH OF THE UNIVERSITY OF WICHITA	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	THE FOUNDATION FOR INDUSTRIAL RESEARCH OF THE UNIVERSITY OF WICHITA .
	manualset3
211167	1	419375	7	NULL	NULL	0	NULL	effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect is mediated through EPOR signaling , since hepcidin mRNA levels are restored by pretreatment with an EPOR-blocking antibody .
	manualset3
211168	2	419375	7	NULL	NULL	0	NULL	EPOR signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect is mediated through EPOR signaling , since hepcidin mRNA levels are restored by pretreatment with an EPOR-blocking antibody .
	manualset3
211169	3	419375	7	NULL	NULL	0	NULL	hepcidin mRNA levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect is mediated through EPOR signaling , since hepcidin mRNA levels are restored by pretreatment with an EPOR-blocking antibody .
	manualset3
211170	4	419375	7	NULL	NULL	0	NULL	 pretreatment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect is mediated through EPOR signaling , since hepcidin mRNA levels are restored by pretreatment with an EPOR-blocking antibody .
	manualset3
211171	5	419375	7	NULL	NULL	0	NULL	EPOR-blocking antibody 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect is mediated through EPOR signaling , since hepcidin mRNA levels are restored by pretreatment with an EPOR-blocking antibody .
	manualset3
211172	1	419376	7	NULL	NULL	0	NULL	Embryological study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Embryological study has not been attempted , but the condition seems to be primarily osteogenic in origin .
	manualset3
211173	2	419376	7	NULL	NULL	0	NULL	condition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Embryological study has not been attempted , but the condition seems to be primarily osteogenic in origin .
	manualset3
211174	3	419376	7	NULL	NULL	0	NULL	 primarily osteogenic	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Embryological study has not been attempted , but the condition seems to be primarily osteogenic in origin .
	manualset3
211175	4	419376	7	NULL	NULL	0	NULL	origin	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Embryological study has not been attempted , but the condition seems to be primarily osteogenic in origin .
	manualset3
211176	1	419377	7	NULL	NULL	0	NULL	Five predicted relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Five predicted relationships between age and intellectual level and 16 Rorschach variables were examined through a cross-sectional analysis of 47 healthy , community-dwelling elderly men and women .
	manualset3
211177	2	419377	7	NULL	NULL	0	NULL	 age	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Five predicted relationships between age and intellectual level and 16 Rorschach variables were examined through a cross-sectional analysis of 47 healthy , community-dwelling elderly men and women .
	manualset3
211178	3	419377	7	NULL	NULL	0	NULL	intellectual level 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Five predicted relationships between age and intellectual level and 16 Rorschach variables were examined through a cross-sectional analysis of 47 healthy , community-dwelling elderly men and women .
	manualset3
211179	4	419377	7	NULL	NULL	0	NULL	16 Rorschach variables	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Five predicted relationships between age and intellectual level and 16 Rorschach variables were examined through a cross-sectional analysis of 47 healthy , community-dwelling elderly men and women .
	manualset3
211180	5	419377	7	NULL	NULL	0	NULL	cross-sectional analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Five predicted relationships between age and intellectual level and 16 Rorschach variables were examined through a cross-sectional analysis of 47 healthy , community-dwelling elderly men and women .
	manualset3
211181	6	419377	7	NULL	NULL	0	NULL	 47 healthy , community-dwelling elderly men 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Five predicted relationships between age and intellectual level and 16 Rorschach variables were examined through a cross-sectional analysis of 47 healthy , community-dwelling elderly men and women .
	manualset3
211182	7	419377	7	NULL	NULL	0	NULL	women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Five predicted relationships between age and intellectual level and 16 Rorschach variables were examined through a cross-sectional analysis of 47 healthy , community-dwelling elderly men and women .
	manualset3
211183	1	419378	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although less pronounced , the results were similar when glucose was injected into the carotid artery toward the brain at a dose that did not modify the peripheral glucose level .
	manualset3
211184	2	419378	7	NULL	NULL	0	NULL	glucose	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Although less pronounced , the results were similar when glucose was injected into the carotid artery toward the brain at a dose that did not modify the peripheral glucose level .
	manualset3
211185	3	419378	7	NULL	NULL	0	NULL	carotid artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although less pronounced , the results were similar when glucose was injected into the carotid artery toward the brain at a dose that did not modify the peripheral glucose level .
	manualset3
211186	4	419378	7	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although less pronounced , the results were similar when glucose was injected into the carotid artery toward the brain at a dose that did not modify the peripheral glucose level .
	manualset3
211187	5	419378	7	NULL	NULL	0	NULL	dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although less pronounced , the results were similar when glucose was injected into the carotid artery toward the brain at a dose that did not modify the peripheral glucose level .
	manualset3
211188	6	419378	7	NULL	NULL	0	NULL	 peripheral glucose level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although less pronounced , the results were similar when glucose was injected into the carotid artery toward the brain at a dose that did not modify the peripheral glucose level .
	manualset3
211189	1	419379	7	NULL	NULL	0	NULL	monoamines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Other monoamines , their metabolites or metabolite/monoamine ratios were not affected .
	manualset3
211190	2	419379	7	NULL	NULL	0	NULL	metabolites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Other monoamines , their metabolites or metabolite/monoamine ratios were not affected .
	manualset3
211191	3	419379	7	NULL	NULL	0	NULL	metabolite/monoamine ratios	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Other monoamines , their metabolites or metabolite/monoamine ratios were not affected .
	manualset3
211192	1	419380	7	NULL	NULL	0	NULL	recombinant lipase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The recombinant lipase was purified to homogeneity using ammonium sulfate precipitation , anion-exchange chromatography ( Poros 20 HQ ) and Sephacryl S-200HR .
	manualset3
211193	2	419380	7	NULL	NULL	0	NULL	ammonium sulfate precipitation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The recombinant lipase was purified to homogeneity using ammonium sulfate precipitation , anion-exchange chromatography ( Poros 20 HQ ) and Sephacryl S-200HR .
	manualset3
211194	3	419380	7	NULL	NULL	0	NULL	anion-exchange chromatography ( Poros 20 HQ ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The recombinant lipase was purified to homogeneity using ammonium sulfate precipitation , anion-exchange chromatography ( Poros 20 HQ ) and Sephacryl S-200HR .
	manualset3
211195	4	419380	7	NULL	NULL	0	NULL	Sephacryl S-200HR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The recombinant lipase was purified to homogeneity using ammonium sulfate precipitation , anion-exchange chromatography ( Poros 20 HQ ) and Sephacryl S-200HR .
	manualset3
211196	1	419381	7	NULL	NULL	0	NULL	browning products 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , there is not yet a consensus that the browning products associated with collagen exclusively comprise advanced Maillard products derived from nonenzymatically glycated residues .
	manualset3
211197	2	419381	7	NULL	NULL	0	NULL	collagen 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , there is not yet a consensus that the browning products associated with collagen exclusively comprise advanced Maillard products derived from nonenzymatically glycated residues .
	manualset3
211198	3	419381	7	NULL	NULL	0	NULL	Maillard products	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , there is not yet a consensus that the browning products associated with collagen exclusively comprise advanced Maillard products derived from nonenzymatically glycated residues .
	manualset3
211199	4	419381	7	NULL	NULL	0	NULL	nonenzymatically glycated residues	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , there is not yet a consensus that the browning products associated with collagen exclusively comprise advanced Maillard products derived from nonenzymatically glycated residues .
	manualset3
211200	1	419382	7	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	It developed during a time when the difference between benignancy and malignancy was not as clear and when patients with benign disease were thought to be at significant risk .
	manualset3
211201	2	419382	7	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	It developed during a time when the difference between benignancy and malignancy was not as clear and when patients with benign disease were thought to be at significant risk .
	manualset3
211202	3	419382	7	NULL	NULL	NULL	NULL	 benignancy	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It developed during a time when the difference between benignancy and malignancy was not as clear and when patients with benign disease were thought to be at significant risk .
	manualset3
211203	4	419382	7	NULL	NULL	NULL	NULL	 malignancy	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It developed during a time when the difference between benignancy and malignancy was not as clear and when patients with benign disease were thought to be at significant risk .
	manualset3
211204	5	419382	7	NULL	NULL	0	NULL	 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It developed during a time when the difference between benignancy and malignancy was not as clear and when patients with benign disease were thought to be at significant risk .
	manualset3
211205	6	419382	7	NULL	NULL	NULL	NULL	benign disease	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It developed during a time when the difference between benignancy and malignancy was not as clear and when patients with benign disease were thought to be at significant risk .
	manualset3
211206	7	419382	7	NULL	NULL	0	NULL	 risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It developed during a time when the difference between benignancy and malignancy was not as clear and when patients with benign disease were thought to be at significant risk .
	manualset3
211207	1	419383	7	NULL	NULL	0	NULL	strongest risk factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the strongest risk factors for colon cancer is age .
	manualset3
211208	2	419383	7	NULL	NULL	0	NULL	colon cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the strongest risk factors for colon cancer is age .
	manualset3
211209	3	419383	7	NULL	NULL	0	NULL	age	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the strongest risk factors for colon cancer is age .
	manualset3
211210	4	419383	7	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the strongest risk factors for colon cancer is age .
	manualset3
211211	1	419384	7	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of recent studies have been performed , concerning 1 ) their overall architecture ; 2 ) migration of B-lymphocytes ; 3 ) localization of accessory cells and T-lymphocytes which are believed to be involved in humoral immune responses ; and 4 ) localization patterns of specific antibody-forming cells developing during thymus dependent and thymus independent immune responses .
	manualset3
211212	2	419384	7	NULL	NULL	0	NULL	recent studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of recent studies have been performed , concerning 1 ) their overall architecture ; 2 ) migration of B-lymphocytes ; 3 ) localization of accessory cells and T-lymphocytes which are believed to be involved in humoral immune responses ; and 4 ) localization patterns of specific antibody-forming cells developing during thymus dependent and thymus independent immune responses .
	manualset3
211213	3	419384	7	NULL	NULL	0	NULL	architecture	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of recent studies have been performed , concerning 1 ) their overall architecture ; 2 ) migration of B-lymphocytes ; 3 ) localization of accessory cells and T-lymphocytes which are believed to be involved in humoral immune responses ; and 4 ) localization patterns of specific antibody-forming cells developing during thymus dependent and thymus independent immune responses .
	manualset3
211214	4	419384	7	NULL	NULL	0	NULL	migration 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of recent studies have been performed , concerning 1 ) their overall architecture ; 2 ) migration of B-lymphocytes ; 3 ) localization of accessory cells and T-lymphocytes which are believed to be involved in humoral immune responses ; and 4 ) localization patterns of specific antibody-forming cells developing during thymus dependent and thymus independent immune responses .
	manualset3
211215	5	419384	7	NULL	NULL	0	NULL	B-lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of recent studies have been performed , concerning 1 ) their overall architecture ; 2 ) migration of B-lymphocytes ; 3 ) localization of accessory cells and T-lymphocytes which are believed to be involved in humoral immune responses ; and 4 ) localization patterns of specific antibody-forming cells developing during thymus dependent and thymus independent immune responses .
	manualset3
211216	6	419384	7	NULL	NULL	0	NULL	localization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of recent studies have been performed , concerning 1 ) their overall architecture ; 2 ) migration of B-lymphocytes ; 3 ) localization of accessory cells and T-lymphocytes which are believed to be involved in humoral immune responses ; and 4 ) localization patterns of specific antibody-forming cells developing during thymus dependent and thymus independent immune responses .
	manualset3
211217	7	419384	7	NULL	NULL	0	NULL	accessory cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of recent studies have been performed , concerning 1 ) their overall architecture ; 2 ) migration of B-lymphocytes ; 3 ) localization of accessory cells and T-lymphocytes which are believed to be involved in humoral immune responses ; and 4 ) localization patterns of specific antibody-forming cells developing during thymus dependent and thymus independent immune responses .
	manualset3
211218	8	419384	7	NULL	NULL	0	NULL	T-lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of recent studies have been performed , concerning 1 ) their overall architecture ; 2 ) migration of B-lymphocytes ; 3 ) localization of accessory cells and T-lymphocytes which are believed to be involved in humoral immune responses ; and 4 ) localization patterns of specific antibody-forming cells developing during thymus dependent and thymus independent immune responses .
	manualset3
211219	9	419384	7	NULL	NULL	0	NULL	humoral immune responses 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of recent studies have been performed , concerning 1 ) their overall architecture ; 2 ) migration of B-lymphocytes ; 3 ) localization of accessory cells and T-lymphocytes which are believed to be involved in humoral immune responses ; and 4 ) localization patterns of specific antibody-forming cells developing during thymus dependent and thymus independent immune responses .
	manualset3
211220	10	419384	7	NULL	NULL	0	NULL	localization patterns	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of recent studies have been performed , concerning 1 ) their overall architecture ; 2 ) migration of B-lymphocytes ; 3 ) localization of accessory cells and T-lymphocytes which are believed to be involved in humoral immune responses ; and 4 ) localization patterns of specific antibody-forming cells developing during thymus dependent and thymus independent immune responses .
	manualset3
211221	11	419384	7	NULL	NULL	0	NULL	antibody-forming cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of recent studies have been performed , concerning 1 ) their overall architecture ; 2 ) migration of B-lymphocytes ; 3 ) localization of accessory cells and T-lymphocytes which are believed to be involved in humoral immune responses ; and 4 ) localization patterns of specific antibody-forming cells developing during thymus dependent and thymus independent immune responses .
	manualset3
211222	12	419384	7	NULL	NULL	0	NULL	 thymus dependent immune responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of recent studies have been performed , concerning 1 ) their overall architecture ; 2 ) migration of B-lymphocytes ; 3 ) localization of accessory cells and T-lymphocytes which are believed to be involved in humoral immune responses ; and 4 ) localization patterns of specific antibody-forming cells developing during thymus dependent and thymus independent immune responses .
	manualset3
211223	13	419384	7	NULL	NULL	0	NULL	 thymus independent immune responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A number of recent studies have been performed , concerning 1 ) their overall architecture ; 2 ) migration of B-lymphocytes ; 3 ) localization of accessory cells and T-lymphocytes which are believed to be involved in humoral immune responses ; and 4 ) localization patterns of specific antibody-forming cells developing during thymus dependent and thymus independent immune responses .
	manualset3
211224	1	419385	7	NULL	NULL	0	NULL	alcohol consumption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Is alcohol consumption associated with gastroesophageal reflux disease ?
	manualset3
211225	2	419385	7	NULL	NULL	0	NULL	gastroesophageal reflux disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Is alcohol consumption associated with gastroesophageal reflux disease ?
	manualset3
211226	1	419386	7	NULL	NULL	0	NULL	Pathology assessment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathology assessment of liver explants in living-donor transplantation programs will provide more precise and reliable information regarding the value of AFP and US as HCC screening tools .
	manualset3
211227	2	419386	7	NULL	NULL	0	NULL	 liver explants	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathology assessment of liver explants in living-donor transplantation programs will provide more precise and reliable information regarding the value of AFP and US as HCC screening tools .
	manualset3
211228	3	419386	7	NULL	NULL	0	NULL	living-donor transplantation programs	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathology assessment of liver explants in living-donor transplantation programs will provide more precise and reliable information regarding the value of AFP and US as HCC screening tools .
	manualset3
211229	4	419386	7	NULL	NULL	0	NULL	information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathology assessment of liver explants in living-donor transplantation programs will provide more precise and reliable information regarding the value of AFP and US as HCC screening tools .
	manualset3
211248	5	419386	7	NULL	NULL	0	NULL	value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathology assessment of liver explants in living-donor transplantation programs will provide more precise and reliable information regarding the value of AFP and US as HCC screening tools .
	manualset3
211249	6	419386	7	NULL	NULL	0	NULL	AFP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathology assessment of liver explants in living-donor transplantation programs will provide more precise and reliable information regarding the value of AFP and US as HCC screening tools .
	manualset3
211250	7	419386	7	NULL	NULL	0	NULL	US	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathology assessment of liver explants in living-donor transplantation programs will provide more precise and reliable information regarding the value of AFP and US as HCC screening tools .
	manualset3
211251	8	419386	7	NULL	NULL	0	NULL	HCC screening tools	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pathology assessment of liver explants in living-donor transplantation programs will provide more precise and reliable information regarding the value of AFP and US as HCC screening tools .
	manualset3
211253	1	419387	7	NULL	NULL	NULL	NULL	Cytogenetics	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Cytogenetics and molecular genetics of hematological malignancy ) .
	manualset3
211255	2	419387	7	NULL	NULL	0	NULL	molecular genetics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cytogenetics and molecular genetics of hematological malignancy ) .
	manualset3
211257	3	419387	7	NULL	NULL	0	NULL	hematological malignancy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cytogenetics and molecular genetics of hematological malignancy ) .
	manualset3
211262	1	419388	7	NULL	NULL	0	NULL	 levels of satisfaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although levels of satisfaction were high , practitioners should be aware of ( a ) potential pressures influencing men to request predictive testing , ( b ) the difficulties that men encounter in establishing surveillance regimens for breast and prostate cancer , and ( c ) the general lack of information about men 's particular experiences in the medical community .
	manualset3
211263	2	419388	7	NULL	NULL	0	NULL	practitioners	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although levels of satisfaction were high , practitioners should be aware of ( a ) potential pressures influencing men to request predictive testing , ( b ) the difficulties that men encounter in establishing surveillance regimens for breast and prostate cancer , and ( c ) the general lack of information about men 's particular experiences in the medical community .
	manualset3
211264	3	419388	7	NULL	NULL	0	NULL	potential pressures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although levels of satisfaction were high , practitioners should be aware of ( a ) potential pressures influencing men to request predictive testing , ( b ) the difficulties that men encounter in establishing surveillance regimens for breast and prostate cancer , and ( c ) the general lack of information about men 's particular experiences in the medical community .
	manualset3
211265	4	419388	7	NULL	NULL	0	NULL	men 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although levels of satisfaction were high , practitioners should be aware of ( a ) potential pressures influencing men to request predictive testing , ( b ) the difficulties that men encounter in establishing surveillance regimens for breast and prostate cancer , and ( c ) the general lack of information about men 's particular experiences in the medical community .
	manualset3
211266	5	419388	7	NULL	NULL	NULL	NULL	predictive testing	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although levels of satisfaction were high , practitioners should be aware of ( a ) potential pressures influencing men to request predictive testing , ( b ) the difficulties that men encounter in establishing surveillance regimens for breast and prostate cancer , and ( c ) the general lack of information about men 's particular experiences in the medical community .
	manualset3
211269	6	419388	7	NULL	NULL	0	NULL	 difficulties	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although levels of satisfaction were high , practitioners should be aware of ( a ) potential pressures influencing men to request predictive testing , ( b ) the difficulties that men encounter in establishing surveillance regimens for breast and prostate cancer , and ( c ) the general lack of information about men 's particular experiences in the medical community .
	manualset3
211271	7	419388	7	NULL	NULL	0	NULL	 men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although levels of satisfaction were high , practitioners should be aware of ( a ) potential pressures influencing men to request predictive testing , ( b ) the difficulties that men encounter in establishing surveillance regimens for breast and prostate cancer , and ( c ) the general lack of information about men 's particular experiences in the medical community .
	manualset3
211272	8	419388	7	NULL	NULL	0	NULL	surveillance regimens 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Although levels of satisfaction were high , practitioners should be aware of ( a ) potential pressures influencing men to request predictive testing , ( b ) the difficulties that men encounter in establishing surveillance regimens for breast and prostate cancer , and ( c ) the general lack of information about men 's particular experiences in the medical community .
	manualset3
211274	9	419388	7	NULL	NULL	0	NULL	breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Although levels of satisfaction were high , practitioners should be aware of ( a ) potential pressures influencing men to request predictive testing , ( b ) the difficulties that men encounter in establishing surveillance regimens for breast and prostate cancer , and ( c ) the general lack of information about men 's particular experiences in the medical community .
	manualset3
211276	10	419388	7	NULL	NULL	0	NULL	prostate cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Although levels of satisfaction were high , practitioners should be aware of ( a ) potential pressures influencing men to request predictive testing , ( b ) the difficulties that men encounter in establishing surveillance regimens for breast and prostate cancer , and ( c ) the general lack of information about men 's particular experiences in the medical community .
	manualset3
211279	11	419388	7	NULL	NULL	0	NULL	lack of information 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Although levels of satisfaction were high , practitioners should be aware of ( a ) potential pressures influencing men to request predictive testing , ( b ) the difficulties that men encounter in establishing surveillance regimens for breast and prostate cancer , and ( c ) the general lack of information about men 's particular experiences in the medical community .
	manualset3
211282	12	419388	7	NULL	NULL	0	NULL	men 's particular experiences	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although levels of satisfaction were high , practitioners should be aware of ( a ) potential pressures influencing men to request predictive testing , ( b ) the difficulties that men encounter in establishing surveillance regimens for breast and prostate cancer , and ( c ) the general lack of information about men 's particular experiences in the medical community .
	manualset3
211283	13	419388	7	NULL	NULL	0	NULL	medical community	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although levels of satisfaction were high , practitioners should be aware of ( a ) potential pressures influencing men to request predictive testing , ( b ) the difficulties that men encounter in establishing surveillance regimens for breast and prostate cancer , and ( c ) the general lack of information about men 's particular experiences in the medical community .
	manualset3
211284	1	419389	7	NULL	NULL	0	NULL	Kinetics	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Kinetics of activation of acetyl-CoA carboxylase by citrate .
	manualset3
211285	2	419389	7	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Kinetics of activation of acetyl-CoA carboxylase by citrate .
	manualset3
211286	3	419389	7	NULL	NULL	0	NULL	acetyl-CoA carboxylase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Kinetics of activation of acetyl-CoA carboxylase by citrate .
	manualset3
211287	4	419389	7	NULL	NULL	0	NULL	 citrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Kinetics of activation of acetyl-CoA carboxylase by citrate .
	manualset3
211288	1	419390	7	NULL	NULL	0	NULL	principal sources	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Generally the principal sources of dental information cited by most mothers were television or radio followed by dentists , school and family .
	manualset3
211289	2	419390	7	NULL	NULL	0	NULL	dental information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Generally the principal sources of dental information cited by most mothers were television or radio followed by dentists , school and family .
	manualset3
211290	3	419390	7	NULL	NULL	0	NULL	mothers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Generally the principal sources of dental information cited by most mothers were television or radio followed by dentists , school and family .
	manualset3
211291	4	419390	7	NULL	NULL	0	NULL	television	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Generally the principal sources of dental information cited by most mothers were television or radio followed by dentists , school and family .
	manualset3
211292	5	419390	7	NULL	NULL	0	NULL	radio	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Generally the principal sources of dental information cited by most mothers were television or radio followed by dentists , school and family .
	manualset3
211293	6	419390	7	NULL	NULL	0	NULL	dentists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Generally the principal sources of dental information cited by most mothers were television or radio followed by dentists , school and family .
	manualset3
211294	7	419390	7	NULL	NULL	0	NULL	school	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Generally the principal sources of dental information cited by most mothers were television or radio followed by dentists , school and family .
	manualset3
211295	8	419390	7	NULL	NULL	0	NULL	 family	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Generally the principal sources of dental information cited by most mothers were television or radio followed by dentists , school and family .
	manualset3
211296	1	419391	7	NULL	NULL	0	NULL	early lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapidly growing , early lesions of pilomatricoma are predominantly composed of basaloid cells and mostly devoid of other diagnostic clues , leading to a false impression of malignancy .
	manualset3
211297	2	419391	7	NULL	NULL	0	NULL	pilomatricoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapidly growing , early lesions of pilomatricoma are predominantly composed of basaloid cells and mostly devoid of other diagnostic clues , leading to a false impression of malignancy .
	manualset3
211298	3	419391	7	NULL	NULL	0	NULL	basaloid cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapidly growing , early lesions of pilomatricoma are predominantly composed of basaloid cells and mostly devoid of other diagnostic clues , leading to a false impression of malignancy .
	manualset3
211299	4	419391	7	NULL	NULL	0	NULL	diagnostic clues	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapidly growing , early lesions of pilomatricoma are predominantly composed of basaloid cells and mostly devoid of other diagnostic clues , leading to a false impression of malignancy .
	manualset3
211300	5	419391	7	NULL	NULL	0	NULL	false impression	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapidly growing , early lesions of pilomatricoma are predominantly composed of basaloid cells and mostly devoid of other diagnostic clues , leading to a false impression of malignancy .
	manualset3
211301	6	419391	7	NULL	NULL	0	NULL	malignancy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Rapidly growing , early lesions of pilomatricoma are predominantly composed of basaloid cells and mostly devoid of other diagnostic clues , leading to a false impression of malignancy .
	manualset3
211302	1	419392	7	NULL	NULL	0	NULL	RO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	RO at non-cytotoxic 1/2000 and 1/1000 dilutions did not affect nitric oxide ( NO ) production by non-stimulated RAW 264.7 cells .
	manualset3
211303	2	419392	7	NULL	NULL	NULL	NULL	non-cytotoxic 1/2000 dilutions	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	RO at non-cytotoxic 1/2000 and 1/1000 dilutions did not affect nitric oxide ( NO ) production by non-stimulated RAW 264.7 cells .
	manualset3
211304	3	419392	7	NULL	NULL	0	NULL	1/1000 dilutions	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	RO at non-cytotoxic 1/2000 and 1/1000 dilutions did not affect nitric oxide ( NO ) production by non-stimulated RAW 264.7 cells .
	manualset3
211305	4	419392	7	NULL	NULL	0	NULL	nitric oxide ( NO ) production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	RO at non-cytotoxic 1/2000 and 1/1000 dilutions did not affect nitric oxide ( NO ) production by non-stimulated RAW 264.7 cells .
	manualset3
211306	5	419392	7	NULL	NULL	0	NULL	non-stimulated RAW 264.7 cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	RO at non-cytotoxic 1/2000 and 1/1000 dilutions did not affect nitric oxide ( NO ) production by non-stimulated RAW 264.7 cells .
	manualset3
211307	1	419393	7	NULL	NULL	0	NULL	proposed integral imaging system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed integral imaging system can display images integrated around three central depth planes by dynamically altering the polarization and controlling both elemental images and dynamic slit array mask accordingly .
	manualset3
211308	2	419393	7	NULL	NULL	0	NULL	images	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed integral imaging system can display images integrated around three central depth planes by dynamically altering the polarization and controlling both elemental images and dynamic slit array mask accordingly .
	manualset3
211309	3	419393	7	NULL	NULL	0	NULL	 three central depth planes	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed integral imaging system can display images integrated around three central depth planes by dynamically altering the polarization and controlling both elemental images and dynamic slit array mask accordingly .
	manualset3
211310	4	419393	7	NULL	NULL	0	NULL	polarization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed integral imaging system can display images integrated around three central depth planes by dynamically altering the polarization and controlling both elemental images and dynamic slit array mask accordingly .
	manualset3
211311	5	419393	7	NULL	NULL	0	NULL	controlling 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed integral imaging system can display images integrated around three central depth planes by dynamically altering the polarization and controlling both elemental images and dynamic slit array mask accordingly .
	manualset3
211312	6	419393	7	NULL	NULL	0	NULL	elemental images	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed integral imaging system can display images integrated around three central depth planes by dynamically altering the polarization and controlling both elemental images and dynamic slit array mask accordingly .
	manualset3
211315	7	419393	7	NULL	NULL	0	NULL	dynamic slit array mask	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed integral imaging system can display images integrated around three central depth planes by dynamically altering the polarization and controlling both elemental images and dynamic slit array mask accordingly .
	manualset3
211321	1	419394	7	NULL	NULL	0	NULL	ErgTx	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	ErgTx recognizes the P-region of HERG channels , blocking the channel function with a K ( d ) in the order of 12 nM .
	manualset3
211322	2	419394	7	NULL	NULL	0	NULL	P-region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	ErgTx recognizes the P-region of HERG channels , blocking the channel function with a K ( d ) in the order of 12 nM .
	manualset3
211323	3	419394	7	NULL	NULL	0	NULL	HERG channels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	ErgTx recognizes the P-region of HERG channels , blocking the channel function with a K ( d ) in the order of 12 nM .
	manualset3
211324	4	419394	7	NULL	NULL	0	NULL	channel function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	ErgTx recognizes the P-region of HERG channels , blocking the channel function with a K ( d ) in the order of 12 nM .
	manualset3
211325	5	419394	7	NULL	NULL	0	NULL	 K ( d )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	ErgTx recognizes the P-region of HERG channels , blocking the channel function with a K ( d ) in the order of 12 nM .
	manualset3
211326	6	419394	7	NULL	NULL	0	NULL	order	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	ErgTx recognizes the P-region of HERG channels , blocking the channel function with a K ( d ) in the order of 12 nM .
	manualset3
211327	7	419394	7	NULL	NULL	0	NULL	12 nM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	ErgTx recognizes the P-region of HERG channels , blocking the channel function with a K ( d ) in the order of 12 nM .
	manualset3
211330	1	419395	7	NULL	NULL	0	NULL	activated human CD4 ( + ) lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using activated human CD4 ( + ) lymphocytes and a peptide array containing 1176 different kinase consensus substrates , we generated a comprehensive profile of GC-induced rapid effects on signal transduction .
	manualset3
211333	2	419395	7	NULL	NULL	0	NULL	peptide array	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using activated human CD4 ( + ) lymphocytes and a peptide array containing 1176 different kinase consensus substrates , we generated a comprehensive profile of GC-induced rapid effects on signal transduction .
	manualset3
211335	3	419395	7	NULL	NULL	0	NULL	1176	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Using activated human CD4 ( + ) lymphocytes and a peptide array containing 1176 different kinase consensus substrates , we generated a comprehensive profile of GC-induced rapid effects on signal transduction .
	manualset3
211336	4	419395	7	NULL	NULL	0	NULL	kinase consensus substrates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using activated human CD4 ( + ) lymphocytes and a peptide array containing 1176 different kinase consensus substrates , we generated a comprehensive profile of GC-induced rapid effects on signal transduction .
	manualset3
211339	5	419395	7	NULL	NULL	0	NULL	comprehensive profile	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using activated human CD4 ( + ) lymphocytes and a peptide array containing 1176 different kinase consensus substrates , we generated a comprehensive profile of GC-induced rapid effects on signal transduction .
	manualset3
211364	6	419395	7	NULL	NULL	0	NULL	GC-induced rapid effects 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using activated human CD4 ( + ) lymphocytes and a peptide array containing 1176 different kinase consensus substrates , we generated a comprehensive profile of GC-induced rapid effects on signal transduction .
	manualset3
211366	7	419395	7	NULL	NULL	0	NULL	signal transduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using activated human CD4 ( + ) lymphocytes and a peptide array containing 1176 different kinase consensus substrates , we generated a comprehensive profile of GC-induced rapid effects on signal transduction .
	manualset3
211465	1	419396	7	NULL	NULL	0	NULL	lower regression rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although lower regression rates were found if women were HPV-positive and had ) or = CIN2 lesions at baseline , effects of condom use were found both in women with CIN1 and in women with ) or = CIN2 lesions .
	manualset3
211466	2	419396	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although lower regression rates were found if women were HPV-positive and had ) or = CIN2 lesions at baseline , effects of condom use were found both in women with CIN1 and in women with ) or = CIN2 lesions .
	manualset3
211467	3	419396	7	NULL	NULL	0	NULL	HPV-positive	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although lower regression rates were found if women were HPV-positive and had ) or = CIN2 lesions at baseline , effects of condom use were found both in women with CIN1 and in women with ) or = CIN2 lesions .
	manualset3
211468	4	419396	7	NULL	NULL	NULL	NULL	CIN2 lesions	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although lower regression rates were found if women were HPV-positive and had ) or = CIN2 lesions at baseline , effects of condom use were found both in women with CIN1 and in women with ) or = CIN2 lesions .
	manualset3
211469	5	419396	7	NULL	NULL	0	NULL	baseline	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although lower regression rates were found if women were HPV-positive and had ) or = CIN2 lesions at baseline , effects of condom use were found both in women with CIN1 and in women with ) or = CIN2 lesions .
	manualset3
211470	6	419396	7	NULL	NULL	NULL	NULL	effects 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although lower regression rates were found if women were HPV-positive and had ) or = CIN2 lesions at baseline , effects of condom use were found both in women with CIN1 and in women with ) or = CIN2 lesions .
	manualset3
211471	7	419396	7	NULL	NULL	0	NULL	 women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although lower regression rates were found if women were HPV-positive and had ) or = CIN2 lesions at baseline , effects of condom use were found both in women with CIN1 and in women with ) or = CIN2 lesions .
	manualset3
211472	8	419396	7	NULL	NULL	0	NULL	CIN1	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Although lower regression rates were found if women were HPV-positive and had ) or = CIN2 lesions at baseline , effects of condom use were found both in women with CIN1 and in women with ) or = CIN2 lesions .
	manualset3
211473	9	419396	7	NULL	NULL	0	NULL	 women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although lower regression rates were found if women were HPV-positive and had ) or = CIN2 lesions at baseline , effects of condom use were found both in women with CIN1 and in women with ) or = CIN2 lesions .
	manualset3
211474	10	419396	7	NULL	NULL	0	NULL	CIN2 lesions	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Although lower regression rates were found if women were HPV-positive and had ) or = CIN2 lesions at baseline , effects of condom use were found both in women with CIN1 and in women with ) or = CIN2 lesions .
	manualset3
211475	11	419396	7	NULL	NULL	0	NULL	condom use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although lower regression rates were found if women were HPV-positive and had ) or = CIN2 lesions at baseline , effects of condom use were found both in women with CIN1 and in women with ) or = CIN2 lesions .
	manualset3
211476	1	419397	7	NULL	NULL	0	NULL	survival-promoting activities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We investigated the survival-promoting activities of muscle - and astrocyte-derived secreted factors and found that astrocyte-conditioned media ( ACM ) was able to save substantially more motoneurons in vitro than muscle-conditioned media ( MCM ) .
	manualset3
211477	2	419397	7	NULL	NULL	0	NULL	muscle -derived secreted factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We investigated the survival-promoting activities of muscle - and astrocyte-derived secreted factors and found that astrocyte-conditioned media ( ACM ) was able to save substantially more motoneurons in vitro than muscle-conditioned media ( MCM ) .
	manualset3
211478	3	419397	7	NULL	NULL	0	NULL	astrocyte-derived secreted factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We investigated the survival-promoting activities of muscle - and astrocyte-derived secreted factors and found that astrocyte-conditioned media ( ACM ) was able to save substantially more motoneurons in vitro than muscle-conditioned media ( MCM ) .
	manualset3
211479	4	419397	7	NULL	NULL	0	NULL	astrocyte-conditioned media ( ACM )	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We investigated the survival-promoting activities of muscle - and astrocyte-derived secreted factors and found that astrocyte-conditioned media ( ACM ) was able to save substantially more motoneurons in vitro than muscle-conditioned media ( MCM ) .
	manualset3
211480	5	419397	7	NULL	NULL	0	NULL	motoneurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We investigated the survival-promoting activities of muscle - and astrocyte-derived secreted factors and found that astrocyte-conditioned media ( ACM ) was able to save substantially more motoneurons in vitro than muscle-conditioned media ( MCM ) .
	manualset3
211481	6	419397	7	NULL	NULL	0	NULL	muscle-conditioned media ( MCM )	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We investigated the survival-promoting activities of muscle - and astrocyte-derived secreted factors and found that astrocyte-conditioned media ( ACM ) was able to save substantially more motoneurons in vitro than muscle-conditioned media ( MCM ) .
	manualset3
211482	1	419398	7	NULL	NULL	0	NULL	Male infertility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Male infertility accounts for ~ 40 % of cases of failure to conceive .
	manualset3
211483	2	419398	7	NULL	NULL	0	NULL	40 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Male infertility accounts for ~ 40 % of cases of failure to conceive .
	manualset3
211484	3	419398	7	NULL	NULL	0	NULL	 cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Male infertility accounts for ~ 40 % of cases of failure to conceive .
	manualset3
211485	4	419398	7	NULL	NULL	0	NULL	failure to conceive	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Male infertility accounts for ~ 40 % of cases of failure to conceive .
	manualset3
211486	1	419399	7	NULL	NULL	0	NULL	 case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of those associated to neuromediator defects .
	manualset3
211487	2	419399	7	NULL	NULL	0	NULL	neuromediator defects	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of those associated to neuromediator defects .
	manualset3
211488	1	419400	7	NULL	NULL	0	NULL	Pressures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pressures of 5x10 ( -10 ) Torr are typical , and the audiofrequency DS measurements can be performed over a range of temperatures 7-500 K , using a continuous-flow cold finger .
	manualset3
211489	2	419400	7	NULL	NULL	0	NULL	5x10 ( -10 ) Torr 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pressures of 5x10 ( -10 ) Torr are typical , and the audiofrequency DS measurements can be performed over a range of temperatures 7-500 K , using a continuous-flow cold finger .
	manualset3
211490	3	419400	7	NULL	NULL	0	NULL	audiofrequency DS measurements	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pressures of 5x10 ( -10 ) Torr are typical , and the audiofrequency DS measurements can be performed over a range of temperatures 7-500 K , using a continuous-flow cold finger .
	manualset3
211491	4	419400	7	NULL	NULL	0	NULL	range of temperatures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pressures of 5x10 ( -10 ) Torr are typical , and the audiofrequency DS measurements can be performed over a range of temperatures 7-500 K , using a continuous-flow cold finger .
	manualset3
211492	5	419400	7	NULL	NULL	0	NULL	7-500 K	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pressures of 5x10 ( -10 ) Torr are typical , and the audiofrequency DS measurements can be performed over a range of temperatures 7-500 K , using a continuous-flow cold finger .
	manualset3
211493	6	419400	7	NULL	NULL	0	NULL	continuous-flow cold finger 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Pressures of 5x10 ( -10 ) Torr are typical , and the audiofrequency DS measurements can be performed over a range of temperatures 7-500 K , using a continuous-flow cold finger .
	manualset3
211494	1	419401	7	NULL	NULL	0	NULL	titanium amide 13	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The titanium amide 13 and all the zirconium amides are active catalysts for the asymmetric hydroamination/cyclization of aminoalkenes , affording cyclic amines in moderate to excellent yields with moderate to excellent ee values ( up to 93 % ) .
	manualset3
211495	2	419401	7	NULL	NULL	0	NULL	zirconium amides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The titanium amide 13 and all the zirconium amides are active catalysts for the asymmetric hydroamination/cyclization of aminoalkenes , affording cyclic amines in moderate to excellent yields with moderate to excellent ee values ( up to 93 % ) .
	manualset3
211496	3	419401	7	NULL	NULL	0	NULL	active catalysts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The titanium amide 13 and all the zirconium amides are active catalysts for the asymmetric hydroamination/cyclization of aminoalkenes , affording cyclic amines in moderate to excellent yields with moderate to excellent ee values ( up to 93 % ) .
	manualset3
211497	4	419401	7	NULL	NULL	0	NULL	asymmetric hydroamination	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The titanium amide 13 and all the zirconium amides are active catalysts for the asymmetric hydroamination/cyclization of aminoalkenes , affording cyclic amines in moderate to excellent yields with moderate to excellent ee values ( up to 93 % ) .
	manualset3
211498	5	419401	7	NULL	NULL	0	NULL	cyclization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The titanium amide 13 and all the zirconium amides are active catalysts for the asymmetric hydroamination/cyclization of aminoalkenes , affording cyclic amines in moderate to excellent yields with moderate to excellent ee values ( up to 93 % ) .
	manualset3
211499	6	419401	7	NULL	NULL	0	NULL	aminoalkenes 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The titanium amide 13 and all the zirconium amides are active catalysts for the asymmetric hydroamination/cyclization of aminoalkenes , affording cyclic amines in moderate to excellent yields with moderate to excellent ee values ( up to 93 % ) .
	manualset3
211500	7	419401	7	NULL	NULL	0	NULL	cyclic amines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The titanium amide 13 and all the zirconium amides are active catalysts for the asymmetric hydroamination/cyclization of aminoalkenes , affording cyclic amines in moderate to excellent yields with moderate to excellent ee values ( up to 93 % ) .
	manualset3
211501	8	419401	7	NULL	NULL	0	NULL	yields 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The titanium amide 13 and all the zirconium amides are active catalysts for the asymmetric hydroamination/cyclization of aminoalkenes , affording cyclic amines in moderate to excellent yields with moderate to excellent ee values ( up to 93 % ) .
	manualset3
211502	9	419401	7	NULL	NULL	0	NULL	ee values 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The titanium amide 13 and all the zirconium amides are active catalysts for the asymmetric hydroamination/cyclization of aminoalkenes , affording cyclic amines in moderate to excellent yields with moderate to excellent ee values ( up to 93 % ) .
	manualset3
211503	10	419401	7	NULL	NULL	0	NULL	 93 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The titanium amide 13 and all the zirconium amides are active catalysts for the asymmetric hydroamination/cyclization of aminoalkenes , affording cyclic amines in moderate to excellent yields with moderate to excellent ee values ( up to 93 % ) .
	manualset3
211504	1	419402	7	NULL	NULL	0	NULL	 Eclampsismus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Eclampsismus during the last war ) .
	manualset3
211505	2	419402	7	NULL	NULL	0	NULL	 last war 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Eclampsismus during the last war ) .
	manualset3
211506	1	419403	7	NULL	NULL	0	NULL	initiation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Most importantly , initiation of transcription from chimeric genes demonstrated the existence of a second promoter located between +464 and +1105 .
	manualset3
211507	2	419403	7	NULL	NULL	0	NULL	transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Most importantly , initiation of transcription from chimeric genes demonstrated the existence of a second promoter located between +464 and +1105 .
	manualset3
211508	3	419403	7	NULL	NULL	0	NULL	 chimeric genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Most importantly , initiation of transcription from chimeric genes demonstrated the existence of a second promoter located between +464 and +1105 .
	manualset3
211509	4	419403	7	NULL	NULL	0	NULL	 existence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Most importantly , initiation of transcription from chimeric genes demonstrated the existence of a second promoter located between +464 and +1105 .
	manualset3
211510	5	419403	7	NULL	NULL	0	NULL	second promoter 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Most importantly , initiation of transcription from chimeric genes demonstrated the existence of a second promoter located between +464 and +1105 .
	manualset3
211511	6	419403	7	NULL	NULL	0	NULL	+464	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Most importantly , initiation of transcription from chimeric genes demonstrated the existence of a second promoter located between +464 and +1105 .
	manualset3
211512	7	419403	7	NULL	NULL	0	NULL	+1105	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Most importantly , initiation of transcription from chimeric genes demonstrated the existence of a second promoter located between +464 and +1105 .
	manualset3
211513	1	419404	7	NULL	NULL	0	NULL	 tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This tumor is generally considered to be of a low grade of malignancy .
	manualset3
211514	2	419404	7	NULL	NULL	0	NULL	low grade	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This tumor is generally considered to be of a low grade of malignancy .
	manualset3
211515	3	419404	7	NULL	NULL	0	NULL	malignancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This tumor is generally considered to be of a low grade of malignancy .
	manualset3
211516	1	419405	7	NULL	NULL	0	NULL	 lower urinary tract complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although lower urinary tract complications have decreased with intermittent catheterization , the effects of increased intravesicular pressure , inflammation , and chronic bacterial colonization or invasion of the urinary tract on long-term renal function are still undetermined .
	manualset3
211517	2	419405	7	NULL	NULL	0	NULL	intermittent catheterization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Although lower urinary tract complications have decreased with intermittent catheterization , the effects of increased intravesicular pressure , inflammation , and chronic bacterial colonization or invasion of the urinary tract on long-term renal function are still undetermined .
	manualset3
211518	3	419405	7	NULL	NULL	0	NULL	 effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although lower urinary tract complications have decreased with intermittent catheterization , the effects of increased intravesicular pressure , inflammation , and chronic bacterial colonization or invasion of the urinary tract on long-term renal function are still undetermined .
	manualset3
211519	4	419405	7	NULL	NULL	0	NULL	increased intravesicular pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although lower urinary tract complications have decreased with intermittent catheterization , the effects of increased intravesicular pressure , inflammation , and chronic bacterial colonization or invasion of the urinary tract on long-term renal function are still undetermined .
	manualset3
211520	5	419405	7	NULL	NULL	0	NULL	 inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although lower urinary tract complications have decreased with intermittent catheterization , the effects of increased intravesicular pressure , inflammation , and chronic bacterial colonization or invasion of the urinary tract on long-term renal function are still undetermined .
	manualset3
211521	6	419405	7	NULL	NULL	0	NULL	chronic bacterial colonization 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although lower urinary tract complications have decreased with intermittent catheterization , the effects of increased intravesicular pressure , inflammation , and chronic bacterial colonization or invasion of the urinary tract on long-term renal function are still undetermined .
	manualset3
211522	7	419405	7	NULL	NULL	0	NULL	invasion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although lower urinary tract complications have decreased with intermittent catheterization , the effects of increased intravesicular pressure , inflammation , and chronic bacterial colonization or invasion of the urinary tract on long-term renal function are still undetermined .
	manualset3
211523	8	419405	7	NULL	NULL	0	NULL	urinary tract 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although lower urinary tract complications have decreased with intermittent catheterization , the effects of increased intravesicular pressure , inflammation , and chronic bacterial colonization or invasion of the urinary tract on long-term renal function are still undetermined .
	manualset3
211524	9	419405	7	NULL	NULL	0	NULL	 long-term renal function 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although lower urinary tract complications have decreased with intermittent catheterization , the effects of increased intravesicular pressure , inflammation , and chronic bacterial colonization or invasion of the urinary tract on long-term renal function are still undetermined .
	manualset3
211525	1	419406	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , purple membranes bound to a lipid bilayer were imaged .
	manualset3
211526	2	419406	7	NULL	NULL	0	NULL	purple membranes	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , purple membranes bound to a lipid bilayer were imaged .
	manualset3
211527	3	419406	7	NULL	NULL	0	NULL	 lipid bilayer	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , purple membranes bound to a lipid bilayer were imaged .
	manualset3
211528	1	419407	7	NULL	NULL	0	NULL	diluted semen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In diluted semen , motility and viability were measured by a computer assisted sperm analyzer ( CASA ; Sperm Vision , Minitb , Germany ) , capacitation and AR were evaluated with a modified chlortetracycline assay ( CTC ) and the AR additionally by flow cytometry .
	manualset3
211529	2	419407	7	NULL	NULL	0	NULL	motility 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In diluted semen , motility and viability were measured by a computer assisted sperm analyzer ( CASA ; Sperm Vision , Minitb , Germany ) , capacitation and AR were evaluated with a modified chlortetracycline assay ( CTC ) and the AR additionally by flow cytometry .
	manualset3
211530	3	419407	7	NULL	NULL	0	NULL	 viability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In diluted semen , motility and viability were measured by a computer assisted sperm analyzer ( CASA ; Sperm Vision , Minitb , Germany ) , capacitation and AR were evaluated with a modified chlortetracycline assay ( CTC ) and the AR additionally by flow cytometry .
	manualset3
211531	4	419407	7	NULL	NULL	0	NULL	computer assisted sperm analyzer	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	In diluted semen , motility and viability were measured by a computer assisted sperm analyzer ( CASA ; Sperm Vision , Minitb , Germany ) , capacitation and AR were evaluated with a modified chlortetracycline assay ( CTC ) and the AR additionally by flow cytometry .
	manualset3
211532	5	419407	7	NULL	NULL	0	NULL	CASA ; Sperm Vision , Minitb , Germany	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	In diluted semen , motility and viability were measured by a computer assisted sperm analyzer ( CASA ; Sperm Vision , Minitb , Germany ) , capacitation and AR were evaluated with a modified chlortetracycline assay ( CTC ) and the AR additionally by flow cytometry .
	manualset3
211533	6	419407	7	NULL	NULL	0	NULL	capacitation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In diluted semen , motility and viability were measured by a computer assisted sperm analyzer ( CASA ; Sperm Vision , Minitb , Germany ) , capacitation and AR were evaluated with a modified chlortetracycline assay ( CTC ) and the AR additionally by flow cytometry .
	manualset3
211534	7	419407	7	NULL	NULL	0	NULL	AR 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In diluted semen , motility and viability were measured by a computer assisted sperm analyzer ( CASA ; Sperm Vision , Minitb , Germany ) , capacitation and AR were evaluated with a modified chlortetracycline assay ( CTC ) and the AR additionally by flow cytometry .
	manualset3
211535	8	419407	7	NULL	NULL	0	NULL	modified chlortetracycline assay ( CTC )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In diluted semen , motility and viability were measured by a computer assisted sperm analyzer ( CASA ; Sperm Vision , Minitb , Germany ) , capacitation and AR were evaluated with a modified chlortetracycline assay ( CTC ) and the AR additionally by flow cytometry .
	manualset3
211536	9	419407	7	NULL	NULL	0	NULL	AR	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In diluted semen , motility and viability were measured by a computer assisted sperm analyzer ( CASA ; Sperm Vision , Minitb , Germany ) , capacitation and AR were evaluated with a modified chlortetracycline assay ( CTC ) and the AR additionally by flow cytometry .
	manualset3
211537	10	419407	7	NULL	NULL	0	NULL	flow cytometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In diluted semen , motility and viability were measured by a computer assisted sperm analyzer ( CASA ; Sperm Vision , Minitb , Germany ) , capacitation and AR were evaluated with a modified chlortetracycline assay ( CTC ) and the AR additionally by flow cytometry .
	manualset3
211554	1	419408	7	NULL	NULL	0	NULL	AP 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	AP is often considered to reflect musical giftedness , but it has also been associated with certain disabilities due to increased prevalence of AP in individuals with sensory and developmental disorders .
	manualset3
211555	2	419408	7	NULL	NULL	0	NULL	musical giftedness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	AP is often considered to reflect musical giftedness , but it has also been associated with certain disabilities due to increased prevalence of AP in individuals with sensory and developmental disorders .
	manualset3
211556	3	419408	7	NULL	NULL	0	NULL	disabilities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	AP is often considered to reflect musical giftedness , but it has also been associated with certain disabilities due to increased prevalence of AP in individuals with sensory and developmental disorders .
	manualset3
211557	4	419408	7	NULL	NULL	0	NULL	 increased prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	AP is often considered to reflect musical giftedness , but it has also been associated with certain disabilities due to increased prevalence of AP in individuals with sensory and developmental disorders .
	manualset3
211558	5	419408	7	NULL	NULL	0	NULL	AP	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	AP is often considered to reflect musical giftedness , but it has also been associated with certain disabilities due to increased prevalence of AP in individuals with sensory and developmental disorders .
	manualset3
211559	6	419408	7	NULL	NULL	0	NULL	 individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	AP is often considered to reflect musical giftedness , but it has also been associated with certain disabilities due to increased prevalence of AP in individuals with sensory and developmental disorders .
	manualset3
211560	7	419408	7	NULL	NULL	0	NULL	sensory disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	AP is often considered to reflect musical giftedness , but it has also been associated with certain disabilities due to increased prevalence of AP in individuals with sensory and developmental disorders .
	manualset3
211561	8	419408	7	NULL	NULL	0	NULL	developmental disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	AP is often considered to reflect musical giftedness , but it has also been associated with certain disabilities due to increased prevalence of AP in individuals with sensory and developmental disorders .
	manualset3
211562	1	419409	7	NULL	NULL	0	NULL	Auxin-binding proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Auxin-binding proteins were photoaffinity labeled by addition of ( 3H ) N3IAA to plasma membrane vesicles prior to exposure to UV light ( 15 sec ; 300 nm ) and detected by subsequent NaDodSO4/PAGE and fluorography .
	manualset3
211563	2	419409	7	NULL	NULL	NULL	NULL	addition	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auxin-binding proteins were photoaffinity labeled by addition of ( 3H ) N3IAA to plasma membrane vesicles prior to exposure to UV light ( 15 sec ; 300 nm ) and detected by subsequent NaDodSO4/PAGE and fluorography .
	manualset3
211564	3	419409	7	NULL	NULL	0	NULL	( 3H ) N3IAA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Auxin-binding proteins were photoaffinity labeled by addition of ( 3H ) N3IAA to plasma membrane vesicles prior to exposure to UV light ( 15 sec ; 300 nm ) and detected by subsequent NaDodSO4/PAGE and fluorography .
	manualset3
211565	4	419409	7	NULL	NULL	0	NULL	plasma membrane vesicles 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Auxin-binding proteins were photoaffinity labeled by addition of ( 3H ) N3IAA to plasma membrane vesicles prior to exposure to UV light ( 15 sec ; 300 nm ) and detected by subsequent NaDodSO4/PAGE and fluorography .
	manualset3
211566	5	419409	7	NULL	NULL	0	NULL	UV light	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Auxin-binding proteins were photoaffinity labeled by addition of ( 3H ) N3IAA to plasma membrane vesicles prior to exposure to UV light ( 15 sec ; 300 nm ) and detected by subsequent NaDodSO4/PAGE and fluorography .
	manualset3
211567	6	419409	7	NULL	NULL	0	NULL	15 sec	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Auxin-binding proteins were photoaffinity labeled by addition of ( 3H ) N3IAA to plasma membrane vesicles prior to exposure to UV light ( 15 sec ; 300 nm ) and detected by subsequent NaDodSO4/PAGE and fluorography .
	manualset3
211568	7	419409	7	NULL	NULL	0	NULL	 300 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Auxin-binding proteins were photoaffinity labeled by addition of ( 3H ) N3IAA to plasma membrane vesicles prior to exposure to UV light ( 15 sec ; 300 nm ) and detected by subsequent NaDodSO4/PAGE and fluorography .
	manualset3
211569	8	419409	7	NULL	NULL	0	NULL	NaDodSO4/PAGE	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Auxin-binding proteins were photoaffinity labeled by addition of ( 3H ) N3IAA to plasma membrane vesicles prior to exposure to UV light ( 15 sec ; 300 nm ) and detected by subsequent NaDodSO4/PAGE and fluorography .
	manualset3
211570	9	419409	7	NULL	NULL	0	NULL	fluorography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Auxin-binding proteins were photoaffinity labeled by addition of ( 3H ) N3IAA to plasma membrane vesicles prior to exposure to UV light ( 15 sec ; 300 nm ) and detected by subsequent NaDodSO4/PAGE and fluorography .
	manualset3
211571	1	419410	7	NULL	NULL	0	NULL	TcYSL7	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	While TcYSL7 was highly expressed in the flowers , TcYSL5 was more highly expressed in the shoots , and the expression of TcYSL3 was equivalent in all the organs tested .
	manualset3
211572	2	419410	7	NULL	NULL	0	NULL	 flowers	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	While TcYSL7 was highly expressed in the flowers , TcYSL5 was more highly expressed in the shoots , and the expression of TcYSL3 was equivalent in all the organs tested .
	manualset3
211573	3	419410	7	NULL	NULL	0	NULL	TcYSL5 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	While TcYSL7 was highly expressed in the flowers , TcYSL5 was more highly expressed in the shoots , and the expression of TcYSL3 was equivalent in all the organs tested .
	manualset3
211574	4	419410	7	NULL	NULL	0	NULL	shoots	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	While TcYSL7 was highly expressed in the flowers , TcYSL5 was more highly expressed in the shoots , and the expression of TcYSL3 was equivalent in all the organs tested .
	manualset3
211575	5	419410	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While TcYSL7 was highly expressed in the flowers , TcYSL5 was more highly expressed in the shoots , and the expression of TcYSL3 was equivalent in all the organs tested .
	manualset3
211576	6	419410	7	NULL	NULL	NULL	NULL	TcYSL3	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	While TcYSL7 was highly expressed in the flowers , TcYSL5 was more highly expressed in the shoots , and the expression of TcYSL3 was equivalent in all the organs tested .
	manualset3
211577	7	419410	7	NULL	NULL	0	NULL	organs 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	While TcYSL7 was highly expressed in the flowers , TcYSL5 was more highly expressed in the shoots , and the expression of TcYSL3 was equivalent in all the organs tested .
	manualset3
211578	1	419411	7	NULL	NULL	0	NULL	changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These changes in the level of mRNA correspond to changes in the activity and amount of acetyl-CoA carboxylase .
	manualset3
211579	2	419411	7	NULL	NULL	0	NULL	 level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These changes in the level of mRNA correspond to changes in the activity and amount of acetyl-CoA carboxylase .
	manualset3
211580	3	419411	7	NULL	NULL	0	NULL	 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	These changes in the level of mRNA correspond to changes in the activity and amount of acetyl-CoA carboxylase .
	manualset3
211581	4	419411	7	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These changes in the level of mRNA correspond to changes in the activity and amount of acetyl-CoA carboxylase .
	manualset3
211582	5	419411	7	NULL	NULL	0	NULL	 amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These changes in the level of mRNA correspond to changes in the activity and amount of acetyl-CoA carboxylase .
	manualset3
211583	6	419411	7	NULL	NULL	0	NULL	 acetyl-CoA carboxylase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These changes in the level of mRNA correspond to changes in the activity and amount of acetyl-CoA carboxylase .
	manualset3
211584	1	419412	7	NULL	NULL	0	NULL	genus Ptilophora	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The genus Ptilophora ( Lepidoptera , Notodontidae ) in China , with description of a new species .
	manualset3
211585	2	419412	7	NULL	NULL	0	NULL	Lepidoptera 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The genus Ptilophora ( Lepidoptera , Notodontidae ) in China , with description of a new species .
	manualset3
211586	3	419412	7	NULL	NULL	0	NULL	Notodontidae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The genus Ptilophora ( Lepidoptera , Notodontidae ) in China , with description of a new species .
	manualset3
211587	4	419412	7	NULL	NULL	0	NULL	China	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The genus Ptilophora ( Lepidoptera , Notodontidae ) in China , with description of a new species .
	manualset3
211588	5	419412	7	NULL	NULL	0	NULL	 description	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The genus Ptilophora ( Lepidoptera , Notodontidae ) in China , with description of a new species .
	manualset3
211589	6	419412	7	NULL	NULL	0	NULL	new species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The genus Ptilophora ( Lepidoptera , Notodontidae ) in China , with description of a new species .
	manualset3
211590	1	419413	7	NULL	NULL	0	NULL	new interesting approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new interesting approach for evaluating some emotional and motivational states in rodents is represented by the measurement of ultrasonic emission in various situations , mainly : by infants when removed from the nest and apparently under stress , cold and/or hunger ; during sexual behavior ; during aggressive encounters ; in response to aversive stimuli .
	manualset3
211591	2	419413	7	NULL	NULL	0	NULL	emotional states	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A new interesting approach for evaluating some emotional and motivational states in rodents is represented by the measurement of ultrasonic emission in various situations , mainly : by infants when removed from the nest and apparently under stress , cold and/or hunger ; during sexual behavior ; during aggressive encounters ; in response to aversive stimuli .
	manualset3
211592	3	419413	7	NULL	NULL	0	NULL	 motivational states	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A new interesting approach for evaluating some emotional and motivational states in rodents is represented by the measurement of ultrasonic emission in various situations , mainly : by infants when removed from the nest and apparently under stress , cold and/or hunger ; during sexual behavior ; during aggressive encounters ; in response to aversive stimuli .
	manualset3
211593	4	419413	7	NULL	NULL	0	NULL	rodents	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A new interesting approach for evaluating some emotional and motivational states in rodents is represented by the measurement of ultrasonic emission in various situations , mainly : by infants when removed from the nest and apparently under stress , cold and/or hunger ; during sexual behavior ; during aggressive encounters ; in response to aversive stimuli .
	manualset3
211594	5	419413	7	NULL	NULL	0	NULL	 measurement	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new interesting approach for evaluating some emotional and motivational states in rodents is represented by the measurement of ultrasonic emission in various situations , mainly : by infants when removed from the nest and apparently under stress , cold and/or hunger ; during sexual behavior ; during aggressive encounters ; in response to aversive stimuli .
	manualset3
211595	6	419413	7	NULL	NULL	0	NULL	ultrasonic emission 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A new interesting approach for evaluating some emotional and motivational states in rodents is represented by the measurement of ultrasonic emission in various situations , mainly : by infants when removed from the nest and apparently under stress , cold and/or hunger ; during sexual behavior ; during aggressive encounters ; in response to aversive stimuli .
	manualset3
211596	7	419413	7	NULL	NULL	0	NULL	situations	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A new interesting approach for evaluating some emotional and motivational states in rodents is represented by the measurement of ultrasonic emission in various situations , mainly : by infants when removed from the nest and apparently under stress , cold and/or hunger ; during sexual behavior ; during aggressive encounters ; in response to aversive stimuli .
	manualset3
211597	8	419413	7	NULL	NULL	0	NULL	infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A new interesting approach for evaluating some emotional and motivational states in rodents is represented by the measurement of ultrasonic emission in various situations , mainly : by infants when removed from the nest and apparently under stress , cold and/or hunger ; during sexual behavior ; during aggressive encounters ; in response to aversive stimuli .
	manualset3
211598	9	419413	7	NULL	NULL	0	NULL	nest	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A new interesting approach for evaluating some emotional and motivational states in rodents is represented by the measurement of ultrasonic emission in various situations , mainly : by infants when removed from the nest and apparently under stress , cold and/or hunger ; during sexual behavior ; during aggressive encounters ; in response to aversive stimuli .
	manualset3
211599	10	419413	7	NULL	NULL	0	NULL	 stress	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A new interesting approach for evaluating some emotional and motivational states in rodents is represented by the measurement of ultrasonic emission in various situations , mainly : by infants when removed from the nest and apparently under stress , cold and/or hunger ; during sexual behavior ; during aggressive encounters ; in response to aversive stimuli .
	manualset3
211600	11	419413	7	NULL	NULL	0	NULL	cold and/or hunger	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A new interesting approach for evaluating some emotional and motivational states in rodents is represented by the measurement of ultrasonic emission in various situations , mainly : by infants when removed from the nest and apparently under stress , cold and/or hunger ; during sexual behavior ; during aggressive encounters ; in response to aversive stimuli .
	manualset3
211601	12	419413	7	NULL	NULL	NULL	NULL	sexual behavior	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A new interesting approach for evaluating some emotional and motivational states in rodents is represented by the measurement of ultrasonic emission in various situations , mainly : by infants when removed from the nest and apparently under stress , cold and/or hunger ; during sexual behavior ; during aggressive encounters ; in response to aversive stimuli .
	manualset3
211602	13	419413	7	NULL	NULL	0	NULL	aggressive encounters 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A new interesting approach for evaluating some emotional and motivational states in rodents is represented by the measurement of ultrasonic emission in various situations , mainly : by infants when removed from the nest and apparently under stress , cold and/or hunger ; during sexual behavior ; during aggressive encounters ; in response to aversive stimuli .
	manualset3
211603	14	419413	7	NULL	NULL	0	NULL	aversive stimuli	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A new interesting approach for evaluating some emotional and motivational states in rodents is represented by the measurement of ultrasonic emission in various situations , mainly : by infants when removed from the nest and apparently under stress , cold and/or hunger ; during sexual behavior ; during aggressive encounters ; in response to aversive stimuli .
	manualset3
211604	1	419414	7	NULL	NULL	0	NULL	evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of the daily food consumption shows that men with higher educational attainment prefer healthier food items than men with lower educational attainment .
	manualset3
211605	2	419414	7	NULL	NULL	0	NULL	daily food consumption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of the daily food consumption shows that men with higher educational attainment prefer healthier food items than men with lower educational attainment .
	manualset3
211606	3	419414	7	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of the daily food consumption shows that men with higher educational attainment prefer healthier food items than men with lower educational attainment .
	manualset3
211607	4	419414	7	NULL	NULL	0	NULL	higher educational attainment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of the daily food consumption shows that men with higher educational attainment prefer healthier food items than men with lower educational attainment .
	manualset3
211608	5	419414	7	NULL	NULL	NULL	NULL	healthier food items	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The evaluation of the daily food consumption shows that men with higher educational attainment prefer healthier food items than men with lower educational attainment .
	manualset3
211609	6	419414	7	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of the daily food consumption shows that men with higher educational attainment prefer healthier food items than men with lower educational attainment .
	manualset3
211610	7	419414	7	NULL	NULL	0	NULL	lower educational attainment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The evaluation of the daily food consumption shows that men with higher educational attainment prefer healthier food items than men with lower educational attainment .
	manualset3
211611	1	419415	7	NULL	NULL	0	NULL	major reforms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although major reforms are underway in many total institutions to humanize treatment procedures , innovative alternatives to custodial care are gaining impetus in the community .
	manualset3
211612	2	419415	7	NULL	NULL	0	NULL	total institutions 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Although major reforms are underway in many total institutions to humanize treatment procedures , innovative alternatives to custodial care are gaining impetus in the community .
	manualset3
211613	3	419415	7	NULL	NULL	0	NULL	treatment procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Although major reforms are underway in many total institutions to humanize treatment procedures , innovative alternatives to custodial care are gaining impetus in the community .
	manualset3
211614	4	419415	7	NULL	NULL	0	NULL	 innovative alternatives	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although major reforms are underway in many total institutions to humanize treatment procedures , innovative alternatives to custodial care are gaining impetus in the community .
	manualset3
211615	5	419415	7	NULL	NULL	0	NULL	 custodial care 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although major reforms are underway in many total institutions to humanize treatment procedures , innovative alternatives to custodial care are gaining impetus in the community .
	manualset3
211616	6	419415	7	NULL	NULL	0	NULL	impetus	process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although major reforms are underway in many total institutions to humanize treatment procedures , innovative alternatives to custodial care are gaining impetus in the community .
	manualset3
211617	7	419415	7	NULL	NULL	0	NULL	community	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although major reforms are underway in many total institutions to humanize treatment procedures , innovative alternatives to custodial care are gaining impetus in the community .
	manualset3
211717	1	419416	7	NULL	NULL	0	NULL	Professional delay	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Professional delay in diagnosing , referring , and appropriately managing of BMS patients occurs frequently .
	manualset3
211718	2	419416	7	NULL	NULL	0	NULL	diagnosing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Professional delay in diagnosing , referring , and appropriately managing of BMS patients occurs frequently .
	manualset3
211719	3	419416	7	NULL	NULL	0	NULL	referring	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Professional delay in diagnosing , referring , and appropriately managing of BMS patients occurs frequently .
	manualset3
211720	4	419416	7	NULL	NULL	0	NULL	managing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Professional delay in diagnosing , referring , and appropriately managing of BMS patients occurs frequently .
	manualset3
211721	5	419416	7	NULL	NULL	0	NULL	BMS patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Professional delay in diagnosing , referring , and appropriately managing of BMS patients occurs frequently .
	manualset3
211722	1	419417	7	NULL	NULL	0	NULL	Opening	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Opening a dental office : selection and hiring of personnel ) .
	manualset3
211723	2	419417	7	NULL	NULL	0	NULL	dental office	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( Opening a dental office : selection and hiring of personnel ) .
	manualset3
211724	3	419417	7	NULL	NULL	0	NULL	 selection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Opening a dental office : selection and hiring of personnel ) .
	manualset3
211725	4	419417	7	NULL	NULL	0	NULL	hiring 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Opening a dental office : selection and hiring of personnel ) .
	manualset3
211726	5	419417	7	NULL	NULL	0	NULL	personnel 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( Opening a dental office : selection and hiring of personnel ) .
	manualset3
211727	1	419418	7	NULL	NULL	NULL	NULL	X-ray absorption edge studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	X-ray absorption edge and extended x-ray absorption fine structure studies have been undertaken on resting ( ferric ) horseradish peroxidase , HRP compound I ( HRP-I ) , HRP compound II ( HRP-II ) , and several highly oxidized synthetic iron porphyrins that may have relevance as models for the iron site in horseradish peroxidase .
	manualset3
211728	2	419418	7	NULL	NULL	0	NULL	extended x-ray absorption fine structure studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray absorption edge and extended x-ray absorption fine structure studies have been undertaken on resting ( ferric ) horseradish peroxidase , HRP compound I ( HRP-I ) , HRP compound II ( HRP-II ) , and several highly oxidized synthetic iron porphyrins that may have relevance as models for the iron site in horseradish peroxidase .
	manualset3
211729	3	419418	7	NULL	NULL	0	NULL	resting ( ferric ) horseradish peroxidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray absorption edge and extended x-ray absorption fine structure studies have been undertaken on resting ( ferric ) horseradish peroxidase , HRP compound I ( HRP-I ) , HRP compound II ( HRP-II ) , and several highly oxidized synthetic iron porphyrins that may have relevance as models for the iron site in horseradish peroxidase .
	manualset3
211730	4	419418	7	NULL	NULL	0	NULL	HRP compound I ( HRP-I )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray absorption edge and extended x-ray absorption fine structure studies have been undertaken on resting ( ferric ) horseradish peroxidase , HRP compound I ( HRP-I ) , HRP compound II ( HRP-II ) , and several highly oxidized synthetic iron porphyrins that may have relevance as models for the iron site in horseradish peroxidase .
	manualset3
211731	5	419418	7	NULL	NULL	0	NULL	HRP compound II ( HRP-II )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray absorption edge and extended x-ray absorption fine structure studies have been undertaken on resting ( ferric ) horseradish peroxidase , HRP compound I ( HRP-I ) , HRP compound II ( HRP-II ) , and several highly oxidized synthetic iron porphyrins that may have relevance as models for the iron site in horseradish peroxidase .
	manualset3
211732	6	419418	7	NULL	NULL	0	NULL	highly oxidized synthetic iron porphyrins 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray absorption edge and extended x-ray absorption fine structure studies have been undertaken on resting ( ferric ) horseradish peroxidase , HRP compound I ( HRP-I ) , HRP compound II ( HRP-II ) , and several highly oxidized synthetic iron porphyrins that may have relevance as models for the iron site in horseradish peroxidase .
	manualset3
211733	7	419418	7	NULL	NULL	0	NULL	models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray absorption edge and extended x-ray absorption fine structure studies have been undertaken on resting ( ferric ) horseradish peroxidase , HRP compound I ( HRP-I ) , HRP compound II ( HRP-II ) , and several highly oxidized synthetic iron porphyrins that may have relevance as models for the iron site in horseradish peroxidase .
	manualset3
211734	8	419418	7	NULL	NULL	0	NULL	iron site 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray absorption edge and extended x-ray absorption fine structure studies have been undertaken on resting ( ferric ) horseradish peroxidase , HRP compound I ( HRP-I ) , HRP compound II ( HRP-II ) , and several highly oxidized synthetic iron porphyrins that may have relevance as models for the iron site in horseradish peroxidase .
	manualset3
211735	9	419418	7	NULL	NULL	0	NULL	horseradish peroxidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray absorption edge and extended x-ray absorption fine structure studies have been undertaken on resting ( ferric ) horseradish peroxidase , HRP compound I ( HRP-I ) , HRP compound II ( HRP-II ) , and several highly oxidized synthetic iron porphyrins that may have relevance as models for the iron site in horseradish peroxidase .
	manualset3
211736	1	419419	7	NULL	NULL	0	NULL	n-3PUFA	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Because this n-3PUFA is most susceptible to lipid peroxidation , mole-rat membranes are substantially more resistant to oxidative stress than are mice membranes .
	manualset3
211737	2	419419	7	NULL	NULL	0	NULL	lipid peroxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Because this n-3PUFA is most susceptible to lipid peroxidation , mole-rat membranes are substantially more resistant to oxidative stress than are mice membranes .
	manualset3
211738	3	419419	7	NULL	NULL	0	NULL	mole-rat membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Because this n-3PUFA is most susceptible to lipid peroxidation , mole-rat membranes are substantially more resistant to oxidative stress than are mice membranes .
	manualset3
211739	4	419419	7	NULL	NULL	0	NULL	oxidative stress	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Because this n-3PUFA is most susceptible to lipid peroxidation , mole-rat membranes are substantially more resistant to oxidative stress than are mice membranes .
	manualset3
211740	5	419419	7	NULL	NULL	0	NULL	mice membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Because this n-3PUFA is most susceptible to lipid peroxidation , mole-rat membranes are substantially more resistant to oxidative stress than are mice membranes .
	manualset3
211741	1	419420	7	NULL	NULL	0	NULL	Working-side tooth contacts	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Working-side tooth contacts included the canine alone , as well as group function , and occlusal loads were progressively shifted toward a posterior contralateral simple balancing contact .
	manualset3
211742	2	419420	7	NULL	NULL	0	NULL	canine	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Working-side tooth contacts included the canine alone , as well as group function , and occlusal loads were progressively shifted toward a posterior contralateral simple balancing contact .
	manualset3
211743	3	419420	7	NULL	NULL	0	NULL	group function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Working-side tooth contacts included the canine alone , as well as group function , and occlusal loads were progressively shifted toward a posterior contralateral simple balancing contact .
	manualset3
211744	4	419420	7	NULL	NULL	0	NULL	 occlusal loads 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Working-side tooth contacts included the canine alone , as well as group function , and occlusal loads were progressively shifted toward a posterior contralateral simple balancing contact .
	manualset3
211745	5	419420	7	NULL	NULL	0	NULL	posterior contralateral simple balancing contact 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Working-side tooth contacts included the canine alone , as well as group function , and occlusal loads were progressively shifted toward a posterior contralateral simple balancing contact .
	manualset3
211746	1	419421	7	NULL	NULL	0	NULL	nonsense mutation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , we identified a nonsense mutation in exon 3 of the patient 's 3beta-hydroxysteroid-delta8 , delta7-isomerase gene .
	manualset3
211747	2	419421	7	NULL	NULL	0	NULL	exon 3	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , we identified a nonsense mutation in exon 3 of the patient 's 3beta-hydroxysteroid-delta8 , delta7-isomerase gene .
	manualset3
211748	3	419421	7	NULL	NULL	0	NULL	patient 's	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , we identified a nonsense mutation in exon 3 of the patient 's 3beta-hydroxysteroid-delta8 , delta7-isomerase gene .
	manualset3
211749	4	419421	7	NULL	NULL	0	NULL	3beta-hydroxysteroid-delta8 , delta7-isomerase gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , we identified a nonsense mutation in exon 3 of the patient 's 3beta-hydroxysteroid-delta8 , delta7-isomerase gene .
	manualset3
211750	1	419422	7	NULL	NULL	0	NULL	report 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report on the clinical and CDKL5 molecular investigation in a very unusual RTT case , with severe , early-neurological involvement in which we have shown in a previous report , a novel P388S MECP2 mutation ( Conforti et al. ( 2003 ) ; Am J Med Genet A 117A : 184-187 ) .
	manualset3
211751	2	419422	7	NULL	NULL	0	NULL	clinical investigation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report on the clinical and CDKL5 molecular investigation in a very unusual RTT case , with severe , early-neurological involvement in which we have shown in a previous report , a novel P388S MECP2 mutation ( Conforti et al. ( 2003 ) ; Am J Med Genet A 117A : 184-187 ) .
	manualset3
211752	3	419422	7	NULL	NULL	0	NULL	CDKL5 molecular investigation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report on the clinical and CDKL5 molecular investigation in a very unusual RTT case , with severe , early-neurological involvement in which we have shown in a previous report , a novel P388S MECP2 mutation ( Conforti et al. ( 2003 ) ; Am J Med Genet A 117A : 184-187 ) .
	manualset3
211753	4	419422	7	NULL	NULL	0	NULL	RTT case	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report on the clinical and CDKL5 molecular investigation in a very unusual RTT case , with severe , early-neurological involvement in which we have shown in a previous report , a novel P388S MECP2 mutation ( Conforti et al. ( 2003 ) ; Am J Med Genet A 117A : 184-187 ) .
	manualset3
211754	5	419422	7	NULL	NULL	0	NULL	early-neurological involvement 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report on the clinical and CDKL5 molecular investigation in a very unusual RTT case , with severe , early-neurological involvement in which we have shown in a previous report , a novel P388S MECP2 mutation ( Conforti et al. ( 2003 ) ; Am J Med Genet A 117A : 184-187 ) .
	manualset3
211755	6	419422	7	NULL	NULL	0	NULL	previous report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report on the clinical and CDKL5 molecular investigation in a very unusual RTT case , with severe , early-neurological involvement in which we have shown in a previous report , a novel P388S MECP2 mutation ( Conforti et al. ( 2003 ) ; Am J Med Genet A 117A : 184-187 ) .
	manualset3
211756	7	419422	7	NULL	NULL	0	NULL	novel P388S MECP2 mutation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report on the clinical and CDKL5 molecular investigation in a very unusual RTT case , with severe , early-neurological involvement in which we have shown in a previous report , a novel P388S MECP2 mutation ( Conforti et al. ( 2003 ) ; Am J Med Genet A 117A : 184-187 ) .
	manualset3
211757	8	419422	7	NULL	NULL	0	NULL	Conforti et al. ( 2003 ) ; Am J Med Genet A 117A : 184-187	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we report on the clinical and CDKL5 molecular investigation in a very unusual RTT case , with severe , early-neurological involvement in which we have shown in a previous report , a novel P388S MECP2 mutation ( Conforti et al. ( 2003 ) ; Am J Med Genet A 117A : 184-187 ) .
	manualset3
211758	1	419423	7	NULL	NULL	0	NULL	Growth arrest	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth arrest can be overridden and cells maintained for a further 11 weeks , by a mitogen mix of fibroblast growth factor 2 , forskolin , and heregulin ( olfactory mitogen medium ) combined with astrocyte-conditioned medium .
	manualset3
211759	2	419423	7	NULL	NULL	0	NULL	 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth arrest can be overridden and cells maintained for a further 11 weeks , by a mitogen mix of fibroblast growth factor 2 , forskolin , and heregulin ( olfactory mitogen medium ) combined with astrocyte-conditioned medium .
	manualset3
211760	3	419423	7	NULL	NULL	0	NULL	11 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth arrest can be overridden and cells maintained for a further 11 weeks , by a mitogen mix of fibroblast growth factor 2 , forskolin , and heregulin ( olfactory mitogen medium ) combined with astrocyte-conditioned medium .
	manualset3
211761	4	419423	7	NULL	NULL	0	NULL	mitogen mix 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth arrest can be overridden and cells maintained for a further 11 weeks , by a mitogen mix of fibroblast growth factor 2 , forskolin , and heregulin ( olfactory mitogen medium ) combined with astrocyte-conditioned medium .
	manualset3
211762	5	419423	7	NULL	NULL	0	NULL	 fibroblast growth factor 2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth arrest can be overridden and cells maintained for a further 11 weeks , by a mitogen mix of fibroblast growth factor 2 , forskolin , and heregulin ( olfactory mitogen medium ) combined with astrocyte-conditioned medium .
	manualset3
211763	6	419423	7	NULL	NULL	0	NULL	 forskolin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth arrest can be overridden and cells maintained for a further 11 weeks , by a mitogen mix of fibroblast growth factor 2 , forskolin , and heregulin ( olfactory mitogen medium ) combined with astrocyte-conditioned medium .
	manualset3
211764	7	419423	7	NULL	NULL	0	NULL	 heregulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth arrest can be overridden and cells maintained for a further 11 weeks , by a mitogen mix of fibroblast growth factor 2 , forskolin , and heregulin ( olfactory mitogen medium ) combined with astrocyte-conditioned medium .
	manualset3
211765	8	419423	7	NULL	NULL	0	NULL	olfactory mitogen medium 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth arrest can be overridden and cells maintained for a further 11 weeks , by a mitogen mix of fibroblast growth factor 2 , forskolin , and heregulin ( olfactory mitogen medium ) combined with astrocyte-conditioned medium .
	manualset3
211766	9	419423	7	NULL	NULL	0	NULL	astrocyte-conditioned medium 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Growth arrest can be overridden and cells maintained for a further 11 weeks , by a mitogen mix of fibroblast growth factor 2 , forskolin , and heregulin ( olfactory mitogen medium ) combined with astrocyte-conditioned medium .
	manualset3
211767	1	419424	7	NULL	NULL	NULL	NULL	 units	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Most units below the ventral hilum of the LSO ( VLPO ) were inhibited by the contralateral stimulus and many were broadly tuned VLPO units produced wide or poorly defined narrow-chopper discharge patterns and intensity functions with high maximum output .
	manualset3
211768	2	419424	7	NULL	NULL	0	NULL	ventral hilum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Most units below the ventral hilum of the LSO ( VLPO ) were inhibited by the contralateral stimulus and many were broadly tuned VLPO units produced wide or poorly defined narrow-chopper discharge patterns and intensity functions with high maximum output .
	manualset3
211769	3	419424	7	NULL	NULL	0	NULL	 LSO	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Most units below the ventral hilum of the LSO ( VLPO ) were inhibited by the contralateral stimulus and many were broadly tuned VLPO units produced wide or poorly defined narrow-chopper discharge patterns and intensity functions with high maximum output .
	manualset3
211770	4	419424	7	NULL	NULL	0	NULL	VLPO	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Most units below the ventral hilum of the LSO ( VLPO ) were inhibited by the contralateral stimulus and many were broadly tuned VLPO units produced wide or poorly defined narrow-chopper discharge patterns and intensity functions with high maximum output .
	manualset3
211771	5	419424	7	NULL	NULL	0	NULL	contralateral stimulus	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Most units below the ventral hilum of the LSO ( VLPO ) were inhibited by the contralateral stimulus and many were broadly tuned VLPO units produced wide or poorly defined narrow-chopper discharge patterns and intensity functions with high maximum output .
	manualset3
211772	6	419424	7	NULL	NULL	0	NULL	VLPO units	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Most units below the ventral hilum of the LSO ( VLPO ) were inhibited by the contralateral stimulus and many were broadly tuned VLPO units produced wide or poorly defined narrow-chopper discharge patterns and intensity functions with high maximum output .
	manualset3
211773	7	419424	7	NULL	NULL	0	NULL	narrow-chopper discharge patterns 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most units below the ventral hilum of the LSO ( VLPO ) were inhibited by the contralateral stimulus and many were broadly tuned VLPO units produced wide or poorly defined narrow-chopper discharge patterns and intensity functions with high maximum output .
	manualset3
211774	8	419424	7	NULL	NULL	0	NULL	intensity functions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most units below the ventral hilum of the LSO ( VLPO ) were inhibited by the contralateral stimulus and many were broadly tuned VLPO units produced wide or poorly defined narrow-chopper discharge patterns and intensity functions with high maximum output .
	manualset3
211775	9	419424	7	NULL	NULL	0	NULL	high maximum output	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Most units below the ventral hilum of the LSO ( VLPO ) were inhibited by the contralateral stimulus and many were broadly tuned VLPO units produced wide or poorly defined narrow-chopper discharge patterns and intensity functions with high maximum output .
	manualset3
211776	1	419425	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Although many cells retain their characteristic neurochemical labeling following ischemia/reperfusion , caution should be used when assuming cells participate in functional retinal circuits based solely on the persistence of neurochemical labeling .
	manualset3
211777	2	419425	7	NULL	NULL	0	NULL	neurochemical labeling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although many cells retain their characteristic neurochemical labeling following ischemia/reperfusion , caution should be used when assuming cells participate in functional retinal circuits based solely on the persistence of neurochemical labeling .
	manualset3
211778	3	419425	7	NULL	NULL	NULL	NULL	ischemia/reperfusion	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although many cells retain their characteristic neurochemical labeling following ischemia/reperfusion , caution should be used when assuming cells participate in functional retinal circuits based solely on the persistence of neurochemical labeling .
	manualset3
211779	4	419425	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Although many cells retain their characteristic neurochemical labeling following ischemia/reperfusion , caution should be used when assuming cells participate in functional retinal circuits based solely on the persistence of neurochemical labeling .
	manualset3
211780	5	419425	7	NULL	NULL	0	NULL	functional retinal circuits 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although many cells retain their characteristic neurochemical labeling following ischemia/reperfusion , caution should be used when assuming cells participate in functional retinal circuits based solely on the persistence of neurochemical labeling .
	manualset3
211781	6	419425	7	NULL	NULL	NULL	NULL	persistence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although many cells retain their characteristic neurochemical labeling following ischemia/reperfusion , caution should be used when assuming cells participate in functional retinal circuits based solely on the persistence of neurochemical labeling .
	manualset3
211782	7	419425	7	NULL	NULL	0	NULL	neurochemical labeling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although many cells retain their characteristic neurochemical labeling following ischemia/reperfusion , caution should be used when assuming cells participate in functional retinal circuits based solely on the persistence of neurochemical labeling .
	manualset3
212958	8	419425	7	NULL	NULL	0	NULL	caution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although many cells retain their characteristic neurochemical labeling following ischemia/reperfusion , caution should be used when assuming cells participate in functional retinal circuits based solely on the persistence of neurochemical labeling .
	manualset3
211783	1	419426	7	NULL	NULL	0	NULL	bronchoconstrictor effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the bronchoconstrictor effect was not blocked by lipoxygenase inhibitors , suggesting the pulmonary effect is not mediated by lipoxygenase products .
	manualset3
211784	2	419426	7	NULL	NULL	0	NULL	lipoxygenase inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the bronchoconstrictor effect was not blocked by lipoxygenase inhibitors , suggesting the pulmonary effect is not mediated by lipoxygenase products .
	manualset3
211785	3	419426	7	NULL	NULL	0	NULL	pulmonary effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the bronchoconstrictor effect was not blocked by lipoxygenase inhibitors , suggesting the pulmonary effect is not mediated by lipoxygenase products .
	manualset3
211786	4	419426	7	NULL	NULL	NULL	NULL	lipoxygenase products	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , the bronchoconstrictor effect was not blocked by lipoxygenase inhibitors , suggesting the pulmonary effect is not mediated by lipoxygenase products .
	manualset3
211787	1	419427	7	NULL	NULL	0	NULL	eukaryotes 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	As in other eukaryotes that have been examined , 5S rRNA is not derived from this precursor molecule .
	manualset3
211788	2	419427	7	NULL	NULL	0	NULL	5S rRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	As in other eukaryotes that have been examined , 5S rRNA is not derived from this precursor molecule .
	manualset3
211789	3	419427	7	NULL	NULL	0	NULL	precursor molecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	As in other eukaryotes that have been examined , 5S rRNA is not derived from this precursor molecule .
	manualset3
211790	1	419428	7	NULL	NULL	0	NULL	Sodium palmitate	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium palmitate and linoleic acid were tested individually to determine the effect of interaction , the fraction free increasing to 2.59 and 1.96 % in the presence of 2 mEq/l of sodium palmitate and linoleic acid , respectively .
	manualset3
211791	2	419428	7	NULL	NULL	0	NULL	linoleic acid	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium palmitate and linoleic acid were tested individually to determine the effect of interaction , the fraction free increasing to 2.59 and 1.96 % in the presence of 2 mEq/l of sodium palmitate and linoleic acid , respectively .
	manualset3
211792	3	419428	7	NULL	NULL	0	NULL	effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium palmitate and linoleic acid were tested individually to determine the effect of interaction , the fraction free increasing to 2.59 and 1.96 % in the presence of 2 mEq/l of sodium palmitate and linoleic acid , respectively .
	manualset3
211793	4	419428	7	NULL	NULL	0	NULL	 interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium palmitate and linoleic acid were tested individually to determine the effect of interaction , the fraction free increasing to 2.59 and 1.96 % in the presence of 2 mEq/l of sodium palmitate and linoleic acid , respectively .
	manualset3
211794	5	419428	7	NULL	NULL	0	NULL	fraction	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium palmitate and linoleic acid were tested individually to determine the effect of interaction , the fraction free increasing to 2.59 and 1.96 % in the presence of 2 mEq/l of sodium palmitate and linoleic acid , respectively .
	manualset3
211795	6	419428	7	NULL	NULL	0	NULL	2.59 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium palmitate and linoleic acid were tested individually to determine the effect of interaction , the fraction free increasing to 2.59 and 1.96 % in the presence of 2 mEq/l of sodium palmitate and linoleic acid , respectively .
	manualset3
211796	7	419428	7	NULL	NULL	0	NULL	1.96 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium palmitate and linoleic acid were tested individually to determine the effect of interaction , the fraction free increasing to 2.59 and 1.96 % in the presence of 2 mEq/l of sodium palmitate and linoleic acid , respectively .
	manualset3
211797	8	419428	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium palmitate and linoleic acid were tested individually to determine the effect of interaction , the fraction free increasing to 2.59 and 1.96 % in the presence of 2 mEq/l of sodium palmitate and linoleic acid , respectively .
	manualset3
211798	9	419428	7	NULL	NULL	0	NULL	2 mEq/l	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium palmitate and linoleic acid were tested individually to determine the effect of interaction , the fraction free increasing to 2.59 and 1.96 % in the presence of 2 mEq/l of sodium palmitate and linoleic acid , respectively .
	manualset3
211799	10	419428	7	NULL	NULL	NULL	NULL	sodium palmitate 	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Sodium palmitate and linoleic acid were tested individually to determine the effect of interaction , the fraction free increasing to 2.59 and 1.96 % in the presence of 2 mEq/l of sodium palmitate and linoleic acid , respectively .
	manualset3
211800	11	419428	7	NULL	NULL	0	NULL	linoleic acid	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sodium palmitate and linoleic acid were tested individually to determine the effect of interaction , the fraction free increasing to 2.59 and 1.96 % in the presence of 2 mEq/l of sodium palmitate and linoleic acid , respectively .
	manualset3
211801	1	419429	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we have estimated the Fe-C-O angles from isotope data in various heme-CO complexes .
	manualset3
211802	2	419429	7	NULL	NULL	0	NULL	Fe-C-O angles	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we have estimated the Fe-C-O angles from isotope data in various heme-CO complexes .
	manualset3
211803	3	419429	7	NULL	NULL	0	NULL	isotope data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we have estimated the Fe-C-O angles from isotope data in various heme-CO complexes .
	manualset3
211804	4	419429	7	NULL	NULL	0	NULL	heme-CO complexes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , we have estimated the Fe-C-O angles from isotope data in various heme-CO complexes .
	manualset3
211805	1	419430	7	NULL	NULL	0	NULL	 surgical procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The surgical procedures were total mastectomy , tonsillectomy and adenoidectomy , placement of a hip prosthesis , and double hernia repair .
	manualset3
211806	2	419430	7	NULL	NULL	0	NULL	 total mastectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The surgical procedures were total mastectomy , tonsillectomy and adenoidectomy , placement of a hip prosthesis , and double hernia repair .
	manualset3
211807	3	419430	7	NULL	NULL	0	NULL	tonsillectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The surgical procedures were total mastectomy , tonsillectomy and adenoidectomy , placement of a hip prosthesis , and double hernia repair .
	manualset3
211808	4	419430	7	NULL	NULL	0	NULL	adenoidectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The surgical procedures were total mastectomy , tonsillectomy and adenoidectomy , placement of a hip prosthesis , and double hernia repair .
	manualset3
211809	5	419430	7	NULL	NULL	0	NULL	placement	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The surgical procedures were total mastectomy , tonsillectomy and adenoidectomy , placement of a hip prosthesis , and double hernia repair .
	manualset3
211810	6	419430	7	NULL	NULL	0	NULL	hip prosthesis	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The surgical procedures were total mastectomy , tonsillectomy and adenoidectomy , placement of a hip prosthesis , and double hernia repair .
	manualset3
211811	7	419430	7	NULL	NULL	0	NULL	double hernia repair	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The surgical procedures were total mastectomy , tonsillectomy and adenoidectomy , placement of a hip prosthesis , and double hernia repair .
	manualset3
211812	1	419431	7	NULL	NULL	0	NULL	effects 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the effects at 45 degrees C , at 39.5 degrees C , neither the inhibition of leucyl-tRNA synthetase activity nor the killing of tsH1 expressed thermotolerance .
	manualset3
211813	2	419431	7	NULL	NULL	0	NULL	45 degrees C	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the effects at 45 degrees C , at 39.5 degrees C , neither the inhibition of leucyl-tRNA synthetase activity nor the killing of tsH1 expressed thermotolerance .
	manualset3
211814	3	419431	7	NULL	NULL	0	NULL	39.5 degrees C	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the effects at 45 degrees C , at 39.5 degrees C , neither the inhibition of leucyl-tRNA synthetase activity nor the killing of tsH1 expressed thermotolerance .
	manualset3
211815	4	419431	7	NULL	NULL	0	NULL	inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the effects at 45 degrees C , at 39.5 degrees C , neither the inhibition of leucyl-tRNA synthetase activity nor the killing of tsH1 expressed thermotolerance .
	manualset3
211816	5	419431	7	NULL	NULL	0	NULL	leucyl-tRNA synthetase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the effects at 45 degrees C , at 39.5 degrees C , neither the inhibition of leucyl-tRNA synthetase activity nor the killing of tsH1 expressed thermotolerance .
	manualset3
211817	6	419431	7	NULL	NULL	0	NULL	killing	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the effects at 45 degrees C , at 39.5 degrees C , neither the inhibition of leucyl-tRNA synthetase activity nor the killing of tsH1 expressed thermotolerance .
	manualset3
211818	7	419431	7	NULL	NULL	0	NULL	tsH1 expressed thermotolerance	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the effects at 45 degrees C , at 39.5 degrees C , neither the inhibition of leucyl-tRNA synthetase activity nor the killing of tsH1 expressed thermotolerance .
	manualset3
211819	1	419432	7	NULL	NULL	0	NULL	Data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Data from a prospective study of a Guatemalan village population revealed an exceedingly high force of infection which may effect nutrition and growth from gestation onward .
	manualset3
211820	2	419432	7	NULL	NULL	0	NULL	 prospective study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Data from a prospective study of a Guatemalan village population revealed an exceedingly high force of infection which may effect nutrition and growth from gestation onward .
	manualset3
211821	3	419432	7	NULL	NULL	0	NULL	Guatemalan village population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Data from a prospective study of a Guatemalan village population revealed an exceedingly high force of infection which may effect nutrition and growth from gestation onward .
	manualset3
211822	4	419432	7	NULL	NULL	0	NULL	high force	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Data from a prospective study of a Guatemalan village population revealed an exceedingly high force of infection which may effect nutrition and growth from gestation onward .
	manualset3
211823	5	419432	7	NULL	NULL	0	NULL	infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Data from a prospective study of a Guatemalan village population revealed an exceedingly high force of infection which may effect nutrition and growth from gestation onward .
	manualset3
211824	6	419432	7	NULL	NULL	0	NULL	nutrition 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Data from a prospective study of a Guatemalan village population revealed an exceedingly high force of infection which may effect nutrition and growth from gestation onward .
	manualset3
211825	7	419432	7	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Data from a prospective study of a Guatemalan village population revealed an exceedingly high force of infection which may effect nutrition and growth from gestation onward .
	manualset3
211826	8	419432	7	NULL	NULL	0	NULL	gestation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Data from a prospective study of a Guatemalan village population revealed an exceedingly high force of infection which may effect nutrition and growth from gestation onward .
	manualset3
211827	1	419433	7	NULL	NULL	0	NULL	Phospholipid transfer protein deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospholipid transfer protein deficiency reduces sperm motility and impairs fertility of mouse males .
	manualset3
211828	2	419433	7	NULL	NULL	0	NULL	sperm motility	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospholipid transfer protein deficiency reduces sperm motility and impairs fertility of mouse males .
	manualset3
211829	3	419433	7	NULL	NULL	0	NULL	fertility	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospholipid transfer protein deficiency reduces sperm motility and impairs fertility of mouse males .
	manualset3
211830	4	419433	7	NULL	NULL	0	NULL	mouse males	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospholipid transfer protein deficiency reduces sperm motility and impairs fertility of mouse males .
	manualset3
211831	1	419434	7	NULL	NULL	0	NULL	Diethylstilboestrol ( DES )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Diethylstilboestrol ( DES ) administered in vivo to 21 day old rats , for up to 4 days , did not significantly alter the expression of either ER as determined by RT-PCR , despite a 5.5-fold increase in granulosa cell number in these ovaries .
	manualset3
211832	2	419434	7	NULL	NULL	0	NULL	21 day	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Diethylstilboestrol ( DES ) administered in vivo to 21 day old rats , for up to 4 days , did not significantly alter the expression of either ER as determined by RT-PCR , despite a 5.5-fold increase in granulosa cell number in these ovaries .
	manualset3
211833	3	419434	7	NULL	NULL	0	NULL	old rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Diethylstilboestrol ( DES ) administered in vivo to 21 day old rats , for up to 4 days , did not significantly alter the expression of either ER as determined by RT-PCR , despite a 5.5-fold increase in granulosa cell number in these ovaries .
	manualset3
211834	4	419434	7	NULL	NULL	0	NULL	4 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Diethylstilboestrol ( DES ) administered in vivo to 21 day old rats , for up to 4 days , did not significantly alter the expression of either ER as determined by RT-PCR , despite a 5.5-fold increase in granulosa cell number in these ovaries .
	manualset3
211835	5	419434	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Diethylstilboestrol ( DES ) administered in vivo to 21 day old rats , for up to 4 days , did not significantly alter the expression of either ER as determined by RT-PCR , despite a 5.5-fold increase in granulosa cell number in these ovaries .
	manualset3
211836	6	419434	7	NULL	NULL	NULL	NULL	ER 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diethylstilboestrol ( DES ) administered in vivo to 21 day old rats , for up to 4 days , did not significantly alter the expression of either ER as determined by RT-PCR , despite a 5.5-fold increase in granulosa cell number in these ovaries .
	manualset3
211837	7	419434	7	NULL	NULL	0	NULL	RT-PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Diethylstilboestrol ( DES ) administered in vivo to 21 day old rats , for up to 4 days , did not significantly alter the expression of either ER as determined by RT-PCR , despite a 5.5-fold increase in granulosa cell number in these ovaries .
	manualset3
211838	8	419434	7	NULL	NULL	0	NULL	5.5-fold increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Diethylstilboestrol ( DES ) administered in vivo to 21 day old rats , for up to 4 days , did not significantly alter the expression of either ER as determined by RT-PCR , despite a 5.5-fold increase in granulosa cell number in these ovaries .
	manualset3
211839	9	419434	7	NULL	NULL	0	NULL	granulosa cell number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Diethylstilboestrol ( DES ) administered in vivo to 21 day old rats , for up to 4 days , did not significantly alter the expression of either ER as determined by RT-PCR , despite a 5.5-fold increase in granulosa cell number in these ovaries .
	manualset3
211840	10	419434	7	NULL	NULL	0	NULL	ovaries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Diethylstilboestrol ( DES ) administered in vivo to 21 day old rats , for up to 4 days , did not significantly alter the expression of either ER as determined by RT-PCR , despite a 5.5-fold increase in granulosa cell number in these ovaries .
	manualset3
211841	1	419435	7	NULL	NULL	0	NULL	Multiple factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple factors are involved in the glutamate-induced excitotoxicity phenomenon , such as overload of ionotropic and metabotropic receptors , excess Ca ( 2 + ) influx , nitric oxide synthase activation , oxidative damage due to increase in free radicals , and release of endogenous polyamine , among others .
	manualset3
211842	2	419435	7	NULL	NULL	0	NULL	glutamate-induced excitotoxicity phenomenon 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple factors are involved in the glutamate-induced excitotoxicity phenomenon , such as overload of ionotropic and metabotropic receptors , excess Ca ( 2 + ) influx , nitric oxide synthase activation , oxidative damage due to increase in free radicals , and release of endogenous polyamine , among others .
	manualset3
211843	3	419435	7	NULL	NULL	0	NULL	overload	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple factors are involved in the glutamate-induced excitotoxicity phenomenon , such as overload of ionotropic and metabotropic receptors , excess Ca ( 2 + ) influx , nitric oxide synthase activation , oxidative damage due to increase in free radicals , and release of endogenous polyamine , among others .
	manualset3
211844	4	419435	7	NULL	NULL	0	NULL	 ionotropic receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple factors are involved in the glutamate-induced excitotoxicity phenomenon , such as overload of ionotropic and metabotropic receptors , excess Ca ( 2 + ) influx , nitric oxide synthase activation , oxidative damage due to increase in free radicals , and release of endogenous polyamine , among others .
	manualset3
211845	5	419435	7	NULL	NULL	0	NULL	metabotropic receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple factors are involved in the glutamate-induced excitotoxicity phenomenon , such as overload of ionotropic and metabotropic receptors , excess Ca ( 2 + ) influx , nitric oxide synthase activation , oxidative damage due to increase in free radicals , and release of endogenous polyamine , among others .
	manualset3
211846	6	419435	7	NULL	NULL	0	NULL	Ca ( 2 + ) influx 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple factors are involved in the glutamate-induced excitotoxicity phenomenon , such as overload of ionotropic and metabotropic receptors , excess Ca ( 2 + ) influx , nitric oxide synthase activation , oxidative damage due to increase in free radicals , and release of endogenous polyamine , among others .
	manualset3
211847	7	419435	7	NULL	NULL	0	NULL	nitric oxide synthase activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple factors are involved in the glutamate-induced excitotoxicity phenomenon , such as overload of ionotropic and metabotropic receptors , excess Ca ( 2 + ) influx , nitric oxide synthase activation , oxidative damage due to increase in free radicals , and release of endogenous polyamine , among others .
	manualset3
211848	8	419435	7	NULL	NULL	0	NULL	oxidative damage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple factors are involved in the glutamate-induced excitotoxicity phenomenon , such as overload of ionotropic and metabotropic receptors , excess Ca ( 2 + ) influx , nitric oxide synthase activation , oxidative damage due to increase in free radicals , and release of endogenous polyamine , among others .
	manualset3
211849	9	419435	7	NULL	NULL	0	NULL	increase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple factors are involved in the glutamate-induced excitotoxicity phenomenon , such as overload of ionotropic and metabotropic receptors , excess Ca ( 2 + ) influx , nitric oxide synthase activation , oxidative damage due to increase in free radicals , and release of endogenous polyamine , among others .
	manualset3
211850	10	419435	7	NULL	NULL	0	NULL	free radicals	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple factors are involved in the glutamate-induced excitotoxicity phenomenon , such as overload of ionotropic and metabotropic receptors , excess Ca ( 2 + ) influx , nitric oxide synthase activation , oxidative damage due to increase in free radicals , and release of endogenous polyamine , among others .
	manualset3
211851	11	419435	7	NULL	NULL	0	NULL	release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple factors are involved in the glutamate-induced excitotoxicity phenomenon , such as overload of ionotropic and metabotropic receptors , excess Ca ( 2 + ) influx , nitric oxide synthase activation , oxidative damage due to increase in free radicals , and release of endogenous polyamine , among others .
	manualset3
211852	12	419435	7	NULL	NULL	0	NULL	endogenous polyamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple factors are involved in the glutamate-induced excitotoxicity phenomenon , such as overload of ionotropic and metabotropic receptors , excess Ca ( 2 + ) influx , nitric oxide synthase activation , oxidative damage due to increase in free radicals , and release of endogenous polyamine , among others .
	manualset3
211853	1	419436	7	NULL	NULL	0	NULL	Bcl-2 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Bcl-2 expression in chronic lymphocytic leukemia and its correlation with the induction of apoptosis and clinical outcome .
	manualset3
211854	2	419436	7	NULL	NULL	0	NULL	chronic lymphocytic leukemia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Bcl-2 expression in chronic lymphocytic leukemia and its correlation with the induction of apoptosis and clinical outcome .
	manualset3
211855	3	419436	7	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Bcl-2 expression in chronic lymphocytic leukemia and its correlation with the induction of apoptosis and clinical outcome .
	manualset3
211856	4	419436	7	NULL	NULL	0	NULL	induction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Bcl-2 expression in chronic lymphocytic leukemia and its correlation with the induction of apoptosis and clinical outcome .
	manualset3
211857	5	419436	7	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Bcl-2 expression in chronic lymphocytic leukemia and its correlation with the induction of apoptosis and clinical outcome .
	manualset3
211858	6	419436	7	NULL	NULL	0	NULL	clinical outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Bcl-2 expression in chronic lymphocytic leukemia and its correlation with the induction of apoptosis and clinical outcome .
	manualset3
211859	1	419437	7	NULL	NULL	0	NULL	complexes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Several complexes of fluorine-substituted phthallic acid anhydrides with chloride anion have been optimized at the RI-MP2 ( full ) / 6-31 + + G ** level of theory .
	manualset3
211860	2	419437	7	NULL	NULL	0	NULL	fluorine-substituted phthallic acid anhydrides 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Several complexes of fluorine-substituted phthallic acid anhydrides with chloride anion have been optimized at the RI-MP2 ( full ) / 6-31 + + G ** level of theory .
	manualset3
211861	3	419437	7	NULL	NULL	0	NULL	chloride anion	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Several complexes of fluorine-substituted phthallic acid anhydrides with chloride anion have been optimized at the RI-MP2 ( full ) / 6-31 + + G ** level of theory .
	manualset3
211862	4	419437	7	NULL	NULL	0	NULL	RI-MP2 ( full ) / 6-31 + + G ** level of theory	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Several complexes of fluorine-substituted phthallic acid anhydrides with chloride anion have been optimized at the RI-MP2 ( full ) / 6-31 + + G ** level of theory .
	manualset3
211863	1	419438	7	NULL	NULL	0	NULL	ROC analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	ROC analysis showed that DXR had an acceptable predictive power in identifying OA patients a low hip BMD ( sensitivity 70 % , specificity 71 % ) .
	manualset3
211864	2	419438	7	NULL	NULL	0	NULL	DXR	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	ROC analysis showed that DXR had an acceptable predictive power in identifying OA patients a low hip BMD ( sensitivity 70 % , specificity 71 % ) .
	manualset3
211865	3	419438	7	NULL	NULL	0	NULL	predictive power	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	ROC analysis showed that DXR had an acceptable predictive power in identifying OA patients a low hip BMD ( sensitivity 70 % , specificity 71 % ) .
	manualset3
211866	4	419438	7	NULL	NULL	0	NULL	 OA patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	ROC analysis showed that DXR had an acceptable predictive power in identifying OA patients a low hip BMD ( sensitivity 70 % , specificity 71 % ) .
	manualset3
211867	5	419438	7	NULL	NULL	0	NULL	low hip BMD	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	ROC analysis showed that DXR had an acceptable predictive power in identifying OA patients a low hip BMD ( sensitivity 70 % , specificity 71 % ) .
	manualset3
211868	6	419438	7	NULL	NULL	0	NULL	sensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	ROC analysis showed that DXR had an acceptable predictive power in identifying OA patients a low hip BMD ( sensitivity 70 % , specificity 71 % ) .
	manualset3
211869	7	419438	7	NULL	NULL	0	NULL	70 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	ROC analysis showed that DXR had an acceptable predictive power in identifying OA patients a low hip BMD ( sensitivity 70 % , specificity 71 % ) .
	manualset3
211870	8	419438	7	NULL	NULL	0	NULL	specificity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	ROC analysis showed that DXR had an acceptable predictive power in identifying OA patients a low hip BMD ( sensitivity 70 % , specificity 71 % ) .
	manualset3
211871	9	419438	7	NULL	NULL	0	NULL	71 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	ROC analysis showed that DXR had an acceptable predictive power in identifying OA patients a low hip BMD ( sensitivity 70 % , specificity 71 % ) .
	manualset3
211872	1	419439	7	NULL	NULL	0	NULL	Superior olivary complex organization	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Superior olivary complex organization and cytoarchitecture may be correlated with function and catarrhine primate phylogeny .
	manualset3
211873	2	419439	7	NULL	NULL	0	NULL	cytoarchitecture	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Superior olivary complex organization and cytoarchitecture may be correlated with function and catarrhine primate phylogeny .
	manualset3
211874	3	419439	7	NULL	NULL	0	NULL	function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Superior olivary complex organization and cytoarchitecture may be correlated with function and catarrhine primate phylogeny .
	manualset3
211875	4	419439	7	NULL	NULL	0	NULL	 catarrhine primate phylogeny	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Superior olivary complex organization and cytoarchitecture may be correlated with function and catarrhine primate phylogeny .
	manualset3
211876	1	419440	7	NULL	NULL	0	NULL	Current management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Current management of nasopharyngeal cancer .
	manualset3
211877	2	419440	7	NULL	NULL	0	NULL	nasopharyngeal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Current management of nasopharyngeal cancer .
	manualset3
211878	1	419441	7	NULL	NULL	0	NULL	Color Doppler ultrasonography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Color and pulsed Doppler ultrasonography was performed in the ophthalmic arteries in each case and the pulsatility index and mean velocity were calculated .
	manualset3
211879	2	419441	7	NULL	NULL	0	NULL	pulsed Doppler ultrasonography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Color and pulsed Doppler ultrasonography was performed in the ophthalmic arteries in each case and the pulsatility index and mean velocity were calculated .
	manualset3
211880	3	419441	7	NULL	NULL	0	NULL	ophthalmic arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Color and pulsed Doppler ultrasonography was performed in the ophthalmic arteries in each case and the pulsatility index and mean velocity were calculated .
	manualset3
211881	4	419441	7	NULL	NULL	0	NULL	case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Color and pulsed Doppler ultrasonography was performed in the ophthalmic arteries in each case and the pulsatility index and mean velocity were calculated .
	manualset3
211882	5	419441	7	NULL	NULL	0	NULL	pulsatility index	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Color and pulsed Doppler ultrasonography was performed in the ophthalmic arteries in each case and the pulsatility index and mean velocity were calculated .
	manualset3
211883	6	419441	7	NULL	NULL	0	NULL	mean velocity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Color and pulsed Doppler ultrasonography was performed in the ophthalmic arteries in each case and the pulsatility index and mean velocity were calculated .
	manualset3
211884	1	419442	7	NULL	NULL	0	NULL	internal lateral nucleus ( IL )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The internal lateral nucleus ( IL ) of the parabrachial nucleus receives information from the spinal cord .
	manualset3
211885	2	419442	7	NULL	NULL	0	NULL	parabrachial nucleus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The internal lateral nucleus ( IL ) of the parabrachial nucleus receives information from the spinal cord .
	manualset3
211886	3	419442	7	NULL	NULL	0	NULL	information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The internal lateral nucleus ( IL ) of the parabrachial nucleus receives information from the spinal cord .
	manualset3
211887	4	419442	7	NULL	NULL	0	NULL	spinal cord	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The internal lateral nucleus ( IL ) of the parabrachial nucleus receives information from the spinal cord .
	manualset3
211888	1	419443	7	NULL	NULL	0	NULL	Proceeding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceeding from an analysis of the results of the comprehensive study of children and adolescents with chronic pulmonary diseases it has been concluded that this method is objective , informative and provides exhaustive information on the state of bronchial permeability and pulmonary-capillary blood flow .
	manualset3
211889	2	419443	7	NULL	NULL	0	NULL	analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceeding from an analysis of the results of the comprehensive study of children and adolescents with chronic pulmonary diseases it has been concluded that this method is objective , informative and provides exhaustive information on the state of bronchial permeability and pulmonary-capillary blood flow .
	manualset3
211890	3	419443	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceeding from an analysis of the results of the comprehensive study of children and adolescents with chronic pulmonary diseases it has been concluded that this method is objective , informative and provides exhaustive information on the state of bronchial permeability and pulmonary-capillary blood flow .
	manualset3
211891	4	419443	7	NULL	NULL	0	NULL	comprehensive study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceeding from an analysis of the results of the comprehensive study of children and adolescents with chronic pulmonary diseases it has been concluded that this method is objective , informative and provides exhaustive information on the state of bronchial permeability and pulmonary-capillary blood flow .
	manualset3
211892	5	419443	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceeding from an analysis of the results of the comprehensive study of children and adolescents with chronic pulmonary diseases it has been concluded that this method is objective , informative and provides exhaustive information on the state of bronchial permeability and pulmonary-capillary blood flow .
	manualset3
211893	6	419443	7	NULL	NULL	0	NULL	adolescents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceeding from an analysis of the results of the comprehensive study of children and adolescents with chronic pulmonary diseases it has been concluded that this method is objective , informative and provides exhaustive information on the state of bronchial permeability and pulmonary-capillary blood flow .
	manualset3
211894	7	419443	7	NULL	NULL	0	NULL	chronic pulmonary diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceeding from an analysis of the results of the comprehensive study of children and adolescents with chronic pulmonary diseases it has been concluded that this method is objective , informative and provides exhaustive information on the state of bronchial permeability and pulmonary-capillary blood flow .
	manualset3
211895	8	419443	7	NULL	NULL	0	NULL	 method 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceeding from an analysis of the results of the comprehensive study of children and adolescents with chronic pulmonary diseases it has been concluded that this method is objective , informative and provides exhaustive information on the state of bronchial permeability and pulmonary-capillary blood flow .
	manualset3
211896	9	419443	7	NULL	NULL	0	NULL	exhaustive information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceeding from an analysis of the results of the comprehensive study of children and adolescents with chronic pulmonary diseases it has been concluded that this method is objective , informative and provides exhaustive information on the state of bronchial permeability and pulmonary-capillary blood flow .
	manualset3
211897	10	419443	7	NULL	NULL	0	NULL	 state 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceeding from an analysis of the results of the comprehensive study of children and adolescents with chronic pulmonary diseases it has been concluded that this method is objective , informative and provides exhaustive information on the state of bronchial permeability and pulmonary-capillary blood flow .
	manualset3
211898	11	419443	7	NULL	NULL	0	NULL	bronchial permeability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceeding from an analysis of the results of the comprehensive study of children and adolescents with chronic pulmonary diseases it has been concluded that this method is objective , informative and provides exhaustive information on the state of bronchial permeability and pulmonary-capillary blood flow .
	manualset3
211899	12	419443	7	NULL	NULL	0	NULL	 pulmonary-capillary blood flow	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceeding from an analysis of the results of the comprehensive study of children and adolescents with chronic pulmonary diseases it has been concluded that this method is objective , informative and provides exhaustive information on the state of bronchial permeability and pulmonary-capillary blood flow .
	manualset3
211900	1	419444	7	NULL	NULL	0	NULL	S. meliloti bdhA mutant	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although many of the S. meliloti bdhA mutant complementing clones restored D-3-hydroxybutyrate dehydrogenase activity to the mutant host , for some of the clones this activity was not detectable .
	manualset3
211901	2	419444	7	NULL	NULL	NULL	NULL	clones 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although many of the S. meliloti bdhA mutant complementing clones restored D-3-hydroxybutyrate dehydrogenase activity to the mutant host , for some of the clones this activity was not detectable .
	manualset3
211902	3	419444	7	NULL	NULL	0	NULL	D-3-hydroxybutyrate dehydrogenase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although many of the S. meliloti bdhA mutant complementing clones restored D-3-hydroxybutyrate dehydrogenase activity to the mutant host , for some of the clones this activity was not detectable .
	manualset3
211903	4	419444	7	NULL	NULL	0	NULL	mutant host	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although many of the S. meliloti bdhA mutant complementing clones restored D-3-hydroxybutyrate dehydrogenase activity to the mutant host , for some of the clones this activity was not detectable .
	manualset3
211904	5	419444	7	NULL	NULL	0	NULL	 clones	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although many of the S. meliloti bdhA mutant complementing clones restored D-3-hydroxybutyrate dehydrogenase activity to the mutant host , for some of the clones this activity was not detectable .
	manualset3
211905	6	419444	7	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although many of the S. meliloti bdhA mutant complementing clones restored D-3-hydroxybutyrate dehydrogenase activity to the mutant host , for some of the clones this activity was not detectable .
	manualset3
211906	1	419445	7	NULL	NULL	0	NULL	randomised study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We conducted a prospective randomised study comparing the clinical , functional and radiographic results of 46 patients treated for scaphoid nonunion using a vascularised bone graft from the dorsal and distal aspect of the radius ( group I ) , relative to 40 patients treated by means of a conventional non-vascularised bone graft from the distal radius ( group II ) .
	manualset3
211907	2	419445	7	NULL	NULL	0	NULL	clinical results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We conducted a prospective randomised study comparing the clinical , functional and radiographic results of 46 patients treated for scaphoid nonunion using a vascularised bone graft from the dorsal and distal aspect of the radius ( group I ) , relative to 40 patients treated by means of a conventional non-vascularised bone graft from the distal radius ( group II ) .
	manualset3
211908	3	419445	7	NULL	NULL	0	NULL	functional results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We conducted a prospective randomised study comparing the clinical , functional and radiographic results of 46 patients treated for scaphoid nonunion using a vascularised bone graft from the dorsal and distal aspect of the radius ( group I ) , relative to 40 patients treated by means of a conventional non-vascularised bone graft from the distal radius ( group II ) .
	manualset3
211909	4	419445	7	NULL	NULL	0	NULL	radiographic results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We conducted a prospective randomised study comparing the clinical , functional and radiographic results of 46 patients treated for scaphoid nonunion using a vascularised bone graft from the dorsal and distal aspect of the radius ( group I ) , relative to 40 patients treated by means of a conventional non-vascularised bone graft from the distal radius ( group II ) .
	manualset3
211910	5	419445	7	NULL	NULL	0	NULL	46 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We conducted a prospective randomised study comparing the clinical , functional and radiographic results of 46 patients treated for scaphoid nonunion using a vascularised bone graft from the dorsal and distal aspect of the radius ( group I ) , relative to 40 patients treated by means of a conventional non-vascularised bone graft from the distal radius ( group II ) .
	manualset3
211911	6	419445	7	NULL	NULL	0	NULL	scaphoid nonunion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We conducted a prospective randomised study comparing the clinical , functional and radiographic results of 46 patients treated for scaphoid nonunion using a vascularised bone graft from the dorsal and distal aspect of the radius ( group I ) , relative to 40 patients treated by means of a conventional non-vascularised bone graft from the distal radius ( group II ) .
	manualset3
211912	7	419445	7	NULL	NULL	NULL	NULL	 vascularised bone graft 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We conducted a prospective randomised study comparing the clinical , functional and radiographic results of 46 patients treated for scaphoid nonunion using a vascularised bone graft from the dorsal and distal aspect of the radius ( group I ) , relative to 40 patients treated by means of a conventional non-vascularised bone graft from the distal radius ( group II ) .
	manualset3
211913	8	419445	7	NULL	NULL	0	NULL	dorsal aspect of the radius	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We conducted a prospective randomised study comparing the clinical , functional and radiographic results of 46 patients treated for scaphoid nonunion using a vascularised bone graft from the dorsal and distal aspect of the radius ( group I ) , relative to 40 patients treated by means of a conventional non-vascularised bone graft from the distal radius ( group II ) .
	manualset3
211914	9	419445	7	NULL	NULL	0	NULL	distal aspect of the radius	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We conducted a prospective randomised study comparing the clinical , functional and radiographic results of 46 patients treated for scaphoid nonunion using a vascularised bone graft from the dorsal and distal aspect of the radius ( group I ) , relative to 40 patients treated by means of a conventional non-vascularised bone graft from the distal radius ( group II ) .
	manualset3
211915	10	419445	7	NULL	NULL	0	NULL	group I	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We conducted a prospective randomised study comparing the clinical , functional and radiographic results of 46 patients treated for scaphoid nonunion using a vascularised bone graft from the dorsal and distal aspect of the radius ( group I ) , relative to 40 patients treated by means of a conventional non-vascularised bone graft from the distal radius ( group II ) .
	manualset3
211916	11	419445	7	NULL	NULL	0	NULL	40 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We conducted a prospective randomised study comparing the clinical , functional and radiographic results of 46 patients treated for scaphoid nonunion using a vascularised bone graft from the dorsal and distal aspect of the radius ( group I ) , relative to 40 patients treated by means of a conventional non-vascularised bone graft from the distal radius ( group II ) .
	manualset3
211917	12	419445	7	NULL	NULL	0	NULL	non-vascularised bone graft	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	We conducted a prospective randomised study comparing the clinical , functional and radiographic results of 46 patients treated for scaphoid nonunion using a vascularised bone graft from the dorsal and distal aspect of the radius ( group I ) , relative to 40 patients treated by means of a conventional non-vascularised bone graft from the distal radius ( group II ) .
	manualset3
211918	13	419445	7	NULL	NULL	0	NULL	distal radius	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We conducted a prospective randomised study comparing the clinical , functional and radiographic results of 46 patients treated for scaphoid nonunion using a vascularised bone graft from the dorsal and distal aspect of the radius ( group I ) , relative to 40 patients treated by means of a conventional non-vascularised bone graft from the distal radius ( group II ) .
	manualset3
211919	14	419445	7	NULL	NULL	0	NULL	group II	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We conducted a prospective randomised study comparing the clinical , functional and radiographic results of 46 patients treated for scaphoid nonunion using a vascularised bone graft from the dorsal and distal aspect of the radius ( group I ) , relative to 40 patients treated by means of a conventional non-vascularised bone graft from the distal radius ( group II ) .
	manualset3
211920	1	419446	7	NULL	NULL	0	NULL	Myeloid engraftment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Myeloid engraftment occurred promptly with absolute neutrophil count ) 500 cells/mm3 on day 15 + / - 5 and all patients displayed 100 % donor chimerism by 2 months post transplant .
	manualset3
211921	2	419446	7	NULL	NULL	0	NULL	absolute neutrophil count	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Myeloid engraftment occurred promptly with absolute neutrophil count ) 500 cells/mm3 on day 15 + / - 5 and all patients displayed 100 % donor chimerism by 2 months post transplant .
	manualset3
211922	3	419446	7	NULL	NULL	0	NULL	500 cells/mm3 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Myeloid engraftment occurred promptly with absolute neutrophil count ) 500 cells/mm3 on day 15 + / - 5 and all patients displayed 100 % donor chimerism by 2 months post transplant .
	manualset3
211923	4	419446	7	NULL	NULL	0	NULL	15 + / - 5	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Myeloid engraftment occurred promptly with absolute neutrophil count ) 500 cells/mm3 on day 15 + / - 5 and all patients displayed 100 % donor chimerism by 2 months post transplant .
	manualset3
211924	5	419446	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Myeloid engraftment occurred promptly with absolute neutrophil count ) 500 cells/mm3 on day 15 + / - 5 and all patients displayed 100 % donor chimerism by 2 months post transplant .
	manualset3
211925	6	419446	7	NULL	NULL	0	NULL	100 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Myeloid engraftment occurred promptly with absolute neutrophil count ) 500 cells/mm3 on day 15 + / - 5 and all patients displayed 100 % donor chimerism by 2 months post transplant .
	manualset3
211926	7	419446	7	NULL	NULL	0	NULL	donor chimerism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Myeloid engraftment occurred promptly with absolute neutrophil count ) 500 cells/mm3 on day 15 + / - 5 and all patients displayed 100 % donor chimerism by 2 months post transplant .
	manualset3
211927	8	419446	7	NULL	NULL	0	NULL	2 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Myeloid engraftment occurred promptly with absolute neutrophil count ) 500 cells/mm3 on day 15 + / - 5 and all patients displayed 100 % donor chimerism by 2 months post transplant .
	manualset3
211928	9	419446	7	NULL	NULL	0	NULL	post transplant	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Myeloid engraftment occurred promptly with absolute neutrophil count ) 500 cells/mm3 on day 15 + / - 5 and all patients displayed 100 % donor chimerism by 2 months post transplant .
	manualset3
211929	1	419447	7	NULL	NULL	0	NULL	current study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current study we have demonstrated the ability of these agents to improve blood glucose homeostasis in three mouse models of type 2 diabetes .
	manualset3
211930	2	419447	7	NULL	NULL	0	NULL	ability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current study we have demonstrated the ability of these agents to improve blood glucose homeostasis in three mouse models of type 2 diabetes .
	manualset3
211931	3	419447	7	NULL	NULL	0	NULL	agents 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current study we have demonstrated the ability of these agents to improve blood glucose homeostasis in three mouse models of type 2 diabetes .
	manualset3
211932	4	419447	7	NULL	NULL	0	NULL	blood glucose homeostasis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current study we have demonstrated the ability of these agents to improve blood glucose homeostasis in three mouse models of type 2 diabetes .
	manualset3
211933	5	419447	7	NULL	NULL	0	NULL	three mouse models	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current study we have demonstrated the ability of these agents to improve blood glucose homeostasis in three mouse models of type 2 diabetes .
	manualset3
211934	6	419447	7	NULL	NULL	0	NULL	 type 2 diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In the current study we have demonstrated the ability of these agents to improve blood glucose homeostasis in three mouse models of type 2 diabetes .
	manualset3
211935	1	419448	7	NULL	NULL	NULL	NULL	Microchimerism	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Microchimerism and transmission of porcine endogenous retrovirus from a pig cell line or specific pathogen-free pig islets to mouse tissues and human cells during xenografts in nude mice .
	manualset3
211936	2	419448	7	NULL	NULL	0	NULL	transmission	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Microchimerism and transmission of porcine endogenous retrovirus from a pig cell line or specific pathogen-free pig islets to mouse tissues and human cells during xenografts in nude mice .
	manualset3
211937	3	419448	7	NULL	NULL	0	NULL	porcine endogenous retrovirus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Microchimerism and transmission of porcine endogenous retrovirus from a pig cell line or specific pathogen-free pig islets to mouse tissues and human cells during xenografts in nude mice .
	manualset3
211938	4	419448	7	NULL	NULL	0	NULL	pig cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Microchimerism and transmission of porcine endogenous retrovirus from a pig cell line or specific pathogen-free pig islets to mouse tissues and human cells during xenografts in nude mice .
	manualset3
211939	5	419448	7	NULL	NULL	0	NULL	pathogen-free pig islets 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Microchimerism and transmission of porcine endogenous retrovirus from a pig cell line or specific pathogen-free pig islets to mouse tissues and human cells during xenografts in nude mice .
	manualset3
211940	6	419448	7	NULL	NULL	0	NULL	mouse tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Microchimerism and transmission of porcine endogenous retrovirus from a pig cell line or specific pathogen-free pig islets to mouse tissues and human cells during xenografts in nude mice .
	manualset3
211941	7	419448	7	NULL	NULL	0	NULL	human cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Microchimerism and transmission of porcine endogenous retrovirus from a pig cell line or specific pathogen-free pig islets to mouse tissues and human cells during xenografts in nude mice .
	manualset3
211942	8	419448	7	NULL	NULL	0	NULL	 xenografts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Microchimerism and transmission of porcine endogenous retrovirus from a pig cell line or specific pathogen-free pig islets to mouse tissues and human cells during xenografts in nude mice .
	manualset3
211943	9	419448	7	NULL	NULL	0	NULL	nude mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Microchimerism and transmission of porcine endogenous retrovirus from a pig cell line or specific pathogen-free pig islets to mouse tissues and human cells during xenografts in nude mice .
	manualset3
211944	1	419449	7	NULL	NULL	0	NULL	Levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of indocyanine green retention at 15 min correlated with the activity of hepatic delta-aminolevulinate synthase ( p less than 0.05 ) .
	manualset3
211945	2	419449	7	NULL	NULL	0	NULL	indocyanine green retention	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of indocyanine green retention at 15 min correlated with the activity of hepatic delta-aminolevulinate synthase ( p less than 0.05 ) .
	manualset3
211946	3	419449	7	NULL	NULL	0	NULL	15 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of indocyanine green retention at 15 min correlated with the activity of hepatic delta-aminolevulinate synthase ( p less than 0.05 ) .
	manualset3
211947	4	419449	7	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of indocyanine green retention at 15 min correlated with the activity of hepatic delta-aminolevulinate synthase ( p less than 0.05 ) .
	manualset3
211948	5	419449	7	NULL	NULL	0	NULL	hepatic delta-aminolevulinate synthase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of indocyanine green retention at 15 min correlated with the activity of hepatic delta-aminolevulinate synthase ( p less than 0.05 ) .
	manualset3
211949	6	419449	7	NULL	NULL	0	NULL	p less than 0.05	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Levels of indocyanine green retention at 15 min correlated with the activity of hepatic delta-aminolevulinate synthase ( p less than 0.05 ) .
	manualset3
211950	1	419450	7	NULL	NULL	0	NULL	Serum pancreatic enzymes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum pancreatic enzymes in the elderly .
	manualset3
211951	1	419451	7	NULL	NULL	0	NULL	 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	This gene contains a 15 bp intron , the presence of which presumably prevented its detection on Southern blots by tRNA hybridisation .
	manualset3
211952	2	419451	7	NULL	NULL	0	NULL	15 bp intron	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	This gene contains a 15 bp intron , the presence of which presumably prevented its detection on Southern blots by tRNA hybridisation .
	manualset3
211953	3	419451	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This gene contains a 15 bp intron , the presence of which presumably prevented its detection on Southern blots by tRNA hybridisation .
	manualset3
211954	4	419451	7	NULL	NULL	0	NULL	detection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This gene contains a 15 bp intron , the presence of which presumably prevented its detection on Southern blots by tRNA hybridisation .
	manualset3
211955	5	419451	7	NULL	NULL	0	NULL	Southern blots	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This gene contains a 15 bp intron , the presence of which presumably prevented its detection on Southern blots by tRNA hybridisation .
	manualset3
211956	6	419451	7	NULL	NULL	0	NULL	tRNA hybridisation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This gene contains a 15 bp intron , the presence of which presumably prevented its detection on Southern blots by tRNA hybridisation .
	manualset3
211957	1	419452	7	NULL	NULL	0	NULL	 3 years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past 3 years , surgery was performed on 149 patients ( 55 children and 94 adults ) , who complained of snoring and symptoms related to the sleep apnea syndrome at Fujita Health University , The Second Hospital .
	manualset3
211958	2	419452	7	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past 3 years , surgery was performed on 149 patients ( 55 children and 94 adults ) , who complained of snoring and symptoms related to the sleep apnea syndrome at Fujita Health University , The Second Hospital .
	manualset3
211959	3	419452	7	NULL	NULL	0	NULL	149 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past 3 years , surgery was performed on 149 patients ( 55 children and 94 adults ) , who complained of snoring and symptoms related to the sleep apnea syndrome at Fujita Health University , The Second Hospital .
	manualset3
211960	4	419452	7	NULL	NULL	0	NULL	55 children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past 3 years , surgery was performed on 149 patients ( 55 children and 94 adults ) , who complained of snoring and symptoms related to the sleep apnea syndrome at Fujita Health University , The Second Hospital .
	manualset3
211961	5	419452	7	NULL	NULL	0	NULL	94 adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past 3 years , surgery was performed on 149 patients ( 55 children and 94 adults ) , who complained of snoring and symptoms related to the sleep apnea syndrome at Fujita Health University , The Second Hospital .
	manualset3
211962	6	419452	7	NULL	NULL	0	NULL	snoring	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past 3 years , surgery was performed on 149 patients ( 55 children and 94 adults ) , who complained of snoring and symptoms related to the sleep apnea syndrome at Fujita Health University , The Second Hospital .
	manualset3
211963	7	419452	7	NULL	NULL	0	NULL	symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past 3 years , surgery was performed on 149 patients ( 55 children and 94 adults ) , who complained of snoring and symptoms related to the sleep apnea syndrome at Fujita Health University , The Second Hospital .
	manualset3
211964	8	419452	7	NULL	NULL	0	NULL	sleep apnea syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past 3 years , surgery was performed on 149 patients ( 55 children and 94 adults ) , who complained of snoring and symptoms related to the sleep apnea syndrome at Fujita Health University , The Second Hospital .
	manualset3
211965	9	419452	7	NULL	NULL	0	NULL	Fujita Health University	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past 3 years , surgery was performed on 149 patients ( 55 children and 94 adults ) , who complained of snoring and symptoms related to the sleep apnea syndrome at Fujita Health University , The Second Hospital .
	manualset3
211966	10	419452	7	NULL	NULL	0	NULL	The Second Hospital 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In the past 3 years , surgery was performed on 149 patients ( 55 children and 94 adults ) , who complained of snoring and symptoms related to the sleep apnea syndrome at Fujita Health University , The Second Hospital .
	manualset3
211967	1	419453	7	NULL	NULL	0	NULL	 NAGS	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In NAGS , three AAK domain dimers are interlinked by their N-terminal helices , conforming a hexameric ring , whereas each GNAT domain sits on the AAK domain of an adjacent dimer .
	manualset3
211968	2	419453	7	NULL	NULL	NULL	NULL	three AAK domain dimers 	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In NAGS , three AAK domain dimers are interlinked by their N-terminal helices , conforming a hexameric ring , whereas each GNAT domain sits on the AAK domain of an adjacent dimer .
	manualset3
211969	3	419453	7	NULL	NULL	0	NULL	N-terminal helices	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In NAGS , three AAK domain dimers are interlinked by their N-terminal helices , conforming a hexameric ring , whereas each GNAT domain sits on the AAK domain of an adjacent dimer .
	manualset3
211970	4	419453	7	NULL	NULL	0	NULL	hexameric ring	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In NAGS , three AAK domain dimers are interlinked by their N-terminal helices , conforming a hexameric ring , whereas each GNAT domain sits on the AAK domain of an adjacent dimer .
	manualset3
211971	5	419453	7	NULL	NULL	0	NULL	 GNAT domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In NAGS , three AAK domain dimers are interlinked by their N-terminal helices , conforming a hexameric ring , whereas each GNAT domain sits on the AAK domain of an adjacent dimer .
	manualset3
211972	6	419453	7	NULL	NULL	0	NULL	AAK domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In NAGS , three AAK domain dimers are interlinked by their N-terminal helices , conforming a hexameric ring , whereas each GNAT domain sits on the AAK domain of an adjacent dimer .
	manualset3
211973	7	419453	7	NULL	NULL	NULL	NULL	dimer	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In NAGS , three AAK domain dimers are interlinked by their N-terminal helices , conforming a hexameric ring , whereas each GNAT domain sits on the AAK domain of an adjacent dimer .
	manualset3
211974	1	419454	7	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , the difference of 6.4 % is attributed to the recipient race effect and the remaining 4.6 % to the center effect .
	manualset3
211975	2	419454	7	NULL	NULL	0	NULL	6.4 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , the difference of 6.4 % is attributed to the recipient race effect and the remaining 4.6 % to the center effect .
	manualset3
211976	3	419454	7	NULL	NULL	0	NULL	recipient race effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , the difference of 6.4 % is attributed to the recipient race effect and the remaining 4.6 % to the center effect .
	manualset3
211977	4	419454	7	NULL	NULL	0	NULL	4.6 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , the difference of 6.4 % is attributed to the recipient race effect and the remaining 4.6 % to the center effect .
	manualset3
211978	5	419454	7	NULL	NULL	0	NULL	center effect 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , the difference of 6.4 % is attributed to the recipient race effect and the remaining 4.6 % to the center effect .
	manualset3
211979	1	419455	7	NULL	NULL	0	NULL	legislation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest changes to the legislation to prevent patients from driving with lower-limb plaster casts or knee braces .
	manualset3
211980	2	419455	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest changes to the legislation to prevent patients from driving with lower-limb plaster casts or knee braces .
	manualset3
211981	3	419455	7	NULL	NULL	0	NULL	driving	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest changes to the legislation to prevent patients from driving with lower-limb plaster casts or knee braces .
	manualset3
211982	4	419455	7	NULL	NULL	0	NULL	lower-limb plaster casts	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest changes to the legislation to prevent patients from driving with lower-limb plaster casts or knee braces .
	manualset3
211983	5	419455	7	NULL	NULL	0	NULL	knee braces	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest changes to the legislation to prevent patients from driving with lower-limb plaster casts or knee braces .
	manualset3
214065	6	419455	7	NULL	NULL	0	NULL	changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest changes to the legislation to prevent patients from driving with lower-limb plaster casts or knee braces .
	manualset3
211984	1	419456	7	NULL	NULL	0	NULL	Nurses 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurses and dietitians differed in the frequency with which they adopted various strategies to manage patients who developed diarrhea during EN .
	manualset3
211985	2	419456	7	NULL	NULL	0	NULL	dietitians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurses and dietitians differed in the frequency with which they adopted various strategies to manage patients who developed diarrhea during EN .
	manualset3
211986	3	419456	7	NULL	NULL	0	NULL	 various strategies	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurses and dietitians differed in the frequency with which they adopted various strategies to manage patients who developed diarrhea during EN .
	manualset3
211987	4	419456	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurses and dietitians differed in the frequency with which they adopted various strategies to manage patients who developed diarrhea during EN .
	manualset3
211988	5	419456	7	NULL	NULL	0	NULL	diarrhea	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurses and dietitians differed in the frequency with which they adopted various strategies to manage patients who developed diarrhea during EN .
	manualset3
211989	6	419456	7	NULL	NULL	0	NULL	EN	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurses and dietitians differed in the frequency with which they adopted various strategies to manage patients who developed diarrhea during EN .
	manualset3
211990	7	419456	7	NULL	NULL	0	NULL	 frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nurses and dietitians differed in the frequency with which they adopted various strategies to manage patients who developed diarrhea during EN .
	manualset3
211991	1	419457	7	NULL	NULL	0	NULL	Bleeding time 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Bleeding time was measured by mesenteric vessel puncture and renal cortex or cuticle incision .
	manualset3
211992	2	419457	7	NULL	NULL	0	NULL	 mesenteric vessel puncture	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Bleeding time was measured by mesenteric vessel puncture and renal cortex or cuticle incision .
	manualset3
211993	3	419457	7	NULL	NULL	0	NULL	renal cortex incision	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Bleeding time was measured by mesenteric vessel puncture and renal cortex or cuticle incision .
	manualset3
211994	4	419457	7	NULL	NULL	0	NULL	cuticle incision	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Bleeding time was measured by mesenteric vessel puncture and renal cortex or cuticle incision .
	manualset3
211995	1	419458	7	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although many studies have failed to show major benefits for laparoscopy in terms of postoperative recovery , it must be remembered that most of these have been of insufficient statistical power to settle the issue .
	manualset3
211996	2	419458	7	NULL	NULL	0	NULL	benefits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although many studies have failed to show major benefits for laparoscopy in terms of postoperative recovery , it must be remembered that most of these have been of insufficient statistical power to settle the issue .
	manualset3
211997	3	419458	7	NULL	NULL	0	NULL	laparoscopy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Although many studies have failed to show major benefits for laparoscopy in terms of postoperative recovery , it must be remembered that most of these have been of insufficient statistical power to settle the issue .
	manualset3
211998	4	419458	7	NULL	NULL	0	NULL	postoperative recovery	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although many studies have failed to show major benefits for laparoscopy in terms of postoperative recovery , it must be remembered that most of these have been of insufficient statistical power to settle the issue .
	manualset3
211999	5	419458	7	NULL	NULL	0	NULL	insufficient statistical power	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Although many studies have failed to show major benefits for laparoscopy in terms of postoperative recovery , it must be remembered that most of these have been of insufficient statistical power to settle the issue .
	manualset3
212000	6	419458	7	NULL	NULL	0	NULL	issue	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although many studies have failed to show major benefits for laparoscopy in terms of postoperative recovery , it must be remembered that most of these have been of insufficient statistical power to settle the issue .
	manualset3
212001	1	419459	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	We present data , obtained by using the mouse model , that show that the OspA response was barely detectable , whereas all animals developed significant anti-P39 titers after exposure to B. burgdorferi-infected ticks .
	manualset3
212002	2	419459	7	NULL	NULL	0	NULL	 mouse model	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We present data , obtained by using the mouse model , that show that the OspA response was barely detectable , whereas all animals developed significant anti-P39 titers after exposure to B. burgdorferi-infected ticks .
	manualset3
212003	3	419459	7	NULL	NULL	0	NULL	OspA response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We present data , obtained by using the mouse model , that show that the OspA response was barely detectable , whereas all animals developed significant anti-P39 titers after exposure to B. burgdorferi-infected ticks .
	manualset3
212004	4	419459	7	NULL	NULL	0	NULL	animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We present data , obtained by using the mouse model , that show that the OspA response was barely detectable , whereas all animals developed significant anti-P39 titers after exposure to B. burgdorferi-infected ticks .
	manualset3
212005	5	419459	7	NULL	NULL	0	NULL	anti-P39 titers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We present data , obtained by using the mouse model , that show that the OspA response was barely detectable , whereas all animals developed significant anti-P39 titers after exposure to B. burgdorferi-infected ticks .
	manualset3
212006	6	419459	7	NULL	NULL	0	NULL	B. burgdorferi-infected ticks	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We present data , obtained by using the mouse model , that show that the OspA response was barely detectable , whereas all animals developed significant anti-P39 titers after exposure to B. burgdorferi-infected ticks .
	manualset3
212007	1	419460	7	NULL	NULL	0	NULL	 availability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The availability of an additional intragenic marker in the PKD1 gene will improve the accuracy of linkage studies in ADPKD families .
	manualset3
212008	2	419460	7	NULL	NULL	0	NULL	intragenic marker	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The availability of an additional intragenic marker in the PKD1 gene will improve the accuracy of linkage studies in ADPKD families .
	manualset3
212009	3	419460	7	NULL	NULL	0	NULL	PKD1 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The availability of an additional intragenic marker in the PKD1 gene will improve the accuracy of linkage studies in ADPKD families .
	manualset3
212010	4	419460	7	NULL	NULL	0	NULL	accuracy	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The availability of an additional intragenic marker in the PKD1 gene will improve the accuracy of linkage studies in ADPKD families .
	manualset3
212011	5	419460	7	NULL	NULL	0	NULL	linkage studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The availability of an additional intragenic marker in the PKD1 gene will improve the accuracy of linkage studies in ADPKD families .
	manualset3
212012	6	419460	7	NULL	NULL	0	NULL	ADPKD families	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The availability of an additional intragenic marker in the PKD1 gene will improve the accuracy of linkage studies in ADPKD families .
	manualset3
212013	1	419461	7	NULL	NULL	NULL	NULL	 full-length immediate-early gene ( IE )	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The full-length immediate-early gene ( IE ) was cloned from a genomic library of this primary rhesus CMV isolate ( RhCMV ) using the African green monkey ( AGM ) CMV IE gene as probe .
	manualset3
212014	2	419461	7	NULL	NULL	0	NULL	genomic library 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The full-length immediate-early gene ( IE ) was cloned from a genomic library of this primary rhesus CMV isolate ( RhCMV ) using the African green monkey ( AGM ) CMV IE gene as probe .
	manualset3
212015	3	419461	7	NULL	NULL	0	NULL	primary rhesus CMV isolate ( RhCMV )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The full-length immediate-early gene ( IE ) was cloned from a genomic library of this primary rhesus CMV isolate ( RhCMV ) using the African green monkey ( AGM ) CMV IE gene as probe .
	manualset3
212016	4	419461	7	NULL	NULL	0	NULL	African green monkey ( AGM ) CMV IE gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The full-length immediate-early gene ( IE ) was cloned from a genomic library of this primary rhesus CMV isolate ( RhCMV ) using the African green monkey ( AGM ) CMV IE gene as probe .
	manualset3
212017	1	419462	7	NULL	NULL	0	NULL	inhibitory mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This inhibitory mechanism involves phosphorylation of cdc2 on tyrosine 15 .
	manualset3
212018	2	419462	7	NULL	NULL	0	NULL	phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This inhibitory mechanism involves phosphorylation of cdc2 on tyrosine 15 .
	manualset3
212019	3	419462	7	NULL	NULL	0	NULL	cdc2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This inhibitory mechanism involves phosphorylation of cdc2 on tyrosine 15 .
	manualset3
212020	4	419462	7	NULL	NULL	0	NULL	tyrosine 15	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	This inhibitory mechanism involves phosphorylation of cdc2 on tyrosine 15 .
	manualset3
212021	1	419463	7	NULL	NULL	0	NULL	Experimental studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Experimental studies of PYP by solution NMR and X-ray crystallography suggest a very flexible protein backbone in the ground as well as in the signaling state .
	manualset3
212022	2	419463	7	NULL	NULL	0	NULL	PYP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Experimental studies of PYP by solution NMR and X-ray crystallography suggest a very flexible protein backbone in the ground as well as in the signaling state .
	manualset3
212023	3	419463	7	NULL	NULL	0	NULL	solution NMR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Experimental studies of PYP by solution NMR and X-ray crystallography suggest a very flexible protein backbone in the ground as well as in the signaling state .
	manualset3
212024	4	419463	7	NULL	NULL	0	NULL	X-ray crystallography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Experimental studies of PYP by solution NMR and X-ray crystallography suggest a very flexible protein backbone in the ground as well as in the signaling state .
	manualset3
212025	5	419463	7	NULL	NULL	0	NULL	flexible protein backbone	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Experimental studies of PYP by solution NMR and X-ray crystallography suggest a very flexible protein backbone in the ground as well as in the signaling state .
	manualset3
212026	6	419463	7	NULL	NULL	NULL	NULL	ground state	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Experimental studies of PYP by solution NMR and X-ray crystallography suggest a very flexible protein backbone in the ground as well as in the signaling state .
	manualset3
212027	7	419463	7	NULL	NULL	NULL	NULL	signaling state	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Experimental studies of PYP by solution NMR and X-ray crystallography suggest a very flexible protein backbone in the ground as well as in the signaling state .
	manualset3
212028	1	419464	7	NULL	NULL	0	NULL	cell adhesion assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In cell adhesion assays on extracellular matrix proteins , the alpha 6-specific GoH3 mAb inhibited binding of SCC to laminin , suggesting that alpha 6 beta 4 may function as a laminin receptor in SCC .
	manualset3
212029	2	419464	7	NULL	NULL	0	NULL	extracellular matrix proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In cell adhesion assays on extracellular matrix proteins , the alpha 6-specific GoH3 mAb inhibited binding of SCC to laminin , suggesting that alpha 6 beta 4 may function as a laminin receptor in SCC .
	manualset3
212030	3	419464	7	NULL	NULL	0	NULL	alpha 6-specific GoH3 mAb	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In cell adhesion assays on extracellular matrix proteins , the alpha 6-specific GoH3 mAb inhibited binding of SCC to laminin , suggesting that alpha 6 beta 4 may function as a laminin receptor in SCC .
	manualset3
212031	4	419464	7	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In cell adhesion assays on extracellular matrix proteins , the alpha 6-specific GoH3 mAb inhibited binding of SCC to laminin , suggesting that alpha 6 beta 4 may function as a laminin receptor in SCC .
	manualset3
212032	5	419464	7	NULL	NULL	NULL	NULL	SCC	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In cell adhesion assays on extracellular matrix proteins , the alpha 6-specific GoH3 mAb inhibited binding of SCC to laminin , suggesting that alpha 6 beta 4 may function as a laminin receptor in SCC .
	manualset3
212033	6	419464	7	NULL	NULL	0	NULL	laminin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In cell adhesion assays on extracellular matrix proteins , the alpha 6-specific GoH3 mAb inhibited binding of SCC to laminin , suggesting that alpha 6 beta 4 may function as a laminin receptor in SCC .
	manualset3
212034	7	419464	7	NULL	NULL	0	NULL	alpha 6 beta 4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In cell adhesion assays on extracellular matrix proteins , the alpha 6-specific GoH3 mAb inhibited binding of SCC to laminin , suggesting that alpha 6 beta 4 may function as a laminin receptor in SCC .
	manualset3
212035	8	419464	7	NULL	NULL	0	NULL	laminin receptor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In cell adhesion assays on extracellular matrix proteins , the alpha 6-specific GoH3 mAb inhibited binding of SCC to laminin , suggesting that alpha 6 beta 4 may function as a laminin receptor in SCC .
	manualset3
212036	9	419464	7	NULL	NULL	0	NULL	SCC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In cell adhesion assays on extracellular matrix proteins , the alpha 6-specific GoH3 mAb inhibited binding of SCC to laminin , suggesting that alpha 6 beta 4 may function as a laminin receptor in SCC .
	manualset3
212037	1	419465	7	NULL	NULL	0	NULL	Molecular basis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular basis for dysfunction of some mutant forms of methylmalonyl-CoA mutase : deductions from the structure of methionine synthase .
	manualset3
212038	2	419465	7	NULL	NULL	NULL	NULL	dysfunction	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Molecular basis for dysfunction of some mutant forms of methylmalonyl-CoA mutase : deductions from the structure of methionine synthase .
	manualset3
212039	3	419465	7	NULL	NULL	0	NULL	mutant forms	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular basis for dysfunction of some mutant forms of methylmalonyl-CoA mutase : deductions from the structure of methionine synthase .
	manualset3
212040	4	419465	7	NULL	NULL	0	NULL	methylmalonyl-CoA mutase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular basis for dysfunction of some mutant forms of methylmalonyl-CoA mutase : deductions from the structure of methionine synthase .
	manualset3
212041	5	419465	7	NULL	NULL	0	NULL	deductions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular basis for dysfunction of some mutant forms of methylmalonyl-CoA mutase : deductions from the structure of methionine synthase .
	manualset3
212042	6	419465	7	NULL	NULL	0	NULL	structure 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular basis for dysfunction of some mutant forms of methylmalonyl-CoA mutase : deductions from the structure of methionine synthase .
	manualset3
212043	7	419465	7	NULL	NULL	0	NULL	methionine synthase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Molecular basis for dysfunction of some mutant forms of methylmalonyl-CoA mutase : deductions from the structure of methionine synthase .
	manualset3
212044	1	419466	7	NULL	NULL	0	NULL	Deletion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Deletion of agouti-related protein blunts ethanol self-administration and binge-like drinking in mice .
	manualset3
212045	2	419466	7	NULL	NULL	0	NULL	agouti-related protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Deletion of agouti-related protein blunts ethanol self-administration and binge-like drinking in mice .
	manualset3
212046	3	419466	7	NULL	NULL	0	NULL	ethanol self-administration	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Deletion of agouti-related protein blunts ethanol self-administration and binge-like drinking in mice .
	manualset3
212047	4	419466	7	NULL	NULL	0	NULL	binge-like drinking	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Deletion of agouti-related protein blunts ethanol self-administration and binge-like drinking in mice .
	manualset3
212048	5	419466	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Deletion of agouti-related protein blunts ethanol self-administration and binge-like drinking in mice .
	manualset3
212049	1	419467	7	NULL	NULL	0	NULL	Genetic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic analysis of developmental stages of the cellular slime mold Dictyostelium purpureum .
	manualset3
212050	2	419467	7	NULL	NULL	0	NULL	developmental stages 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic analysis of developmental stages of the cellular slime mold Dictyostelium purpureum .
	manualset3
212051	3	419467	7	NULL	NULL	0	NULL	cellular slime mold Dictyostelium purpureum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic analysis of developmental stages of the cellular slime mold Dictyostelium purpureum .
	manualset3
212052	1	419468	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Although many treatments exist , no one approach corrects all the deficits associated with the loss of orbicularis oculi function .
	manualset3
212053	2	419468	7	NULL	NULL	0	NULL	no one approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although many treatments exist , no one approach corrects all the deficits associated with the loss of orbicularis oculi function .
	manualset3
212054	3	419468	7	NULL	NULL	0	NULL	deficits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although many treatments exist , no one approach corrects all the deficits associated with the loss of orbicularis oculi function .
	manualset3
212055	4	419468	7	NULL	NULL	0	NULL	 loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although many treatments exist , no one approach corrects all the deficits associated with the loss of orbicularis oculi function .
	manualset3
212056	5	419468	7	NULL	NULL	0	NULL	 orbicularis oculi function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although many treatments exist , no one approach corrects all the deficits associated with the loss of orbicularis oculi function .
	manualset3
212057	1	419469	7	NULL	NULL	0	NULL	present method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present method showed significantly high sensitivity and wide dynamic range ; the detection limit for cytochrome c was 6 x 10 ( -9 ) M and the linear dynamic range was greater than two-orders of magnitude ( up to 2 x 10 ( -6 ) M ) .
	manualset3
212058	2	419469	7	NULL	NULL	0	NULL	 high sensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present method showed significantly high sensitivity and wide dynamic range ; the detection limit for cytochrome c was 6 x 10 ( -9 ) M and the linear dynamic range was greater than two-orders of magnitude ( up to 2 x 10 ( -6 ) M ) .
	manualset3
212059	3	419469	7	NULL	NULL	0	NULL	 wide dynamic range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present method showed significantly high sensitivity and wide dynamic range ; the detection limit for cytochrome c was 6 x 10 ( -9 ) M and the linear dynamic range was greater than two-orders of magnitude ( up to 2 x 10 ( -6 ) M ) .
	manualset3
212060	4	419469	7	NULL	NULL	0	NULL	detection limit	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present method showed significantly high sensitivity and wide dynamic range ; the detection limit for cytochrome c was 6 x 10 ( -9 ) M and the linear dynamic range was greater than two-orders of magnitude ( up to 2 x 10 ( -6 ) M ) .
	manualset3
212061	5	419469	7	NULL	NULL	0	NULL	cytochrome c	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present method showed significantly high sensitivity and wide dynamic range ; the detection limit for cytochrome c was 6 x 10 ( -9 ) M and the linear dynamic range was greater than two-orders of magnitude ( up to 2 x 10 ( -6 ) M ) .
	manualset3
212062	6	419469	7	NULL	NULL	0	NULL	6 x 10 ( -9 ) M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The present method showed significantly high sensitivity and wide dynamic range ; the detection limit for cytochrome c was 6 x 10 ( -9 ) M and the linear dynamic range was greater than two-orders of magnitude ( up to 2 x 10 ( -6 ) M ) .
	manualset3
212063	7	419469	7	NULL	NULL	0	NULL	 linear dynamic range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present method showed significantly high sensitivity and wide dynamic range ; the detection limit for cytochrome c was 6 x 10 ( -9 ) M and the linear dynamic range was greater than two-orders of magnitude ( up to 2 x 10 ( -6 ) M ) .
	manualset3
212064	8	419469	7	NULL	NULL	NULL	NULL	two-orders of magnitude	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present method showed significantly high sensitivity and wide dynamic range ; the detection limit for cytochrome c was 6 x 10 ( -9 ) M and the linear dynamic range was greater than two-orders of magnitude ( up to 2 x 10 ( -6 ) M ) .
	manualset3
212065	9	419469	7	NULL	NULL	0	NULL	2 x 10 ( -6 ) M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The present method showed significantly high sensitivity and wide dynamic range ; the detection limit for cytochrome c was 6 x 10 ( -9 ) M and the linear dynamic range was greater than two-orders of magnitude ( up to 2 x 10 ( -6 ) M ) .
	manualset3
212066	1	419470	7	NULL	NULL	0	NULL	Hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypertension is prevalent in 49 % of renal transplant recipients .
	manualset3
212067	2	419470	7	NULL	NULL	0	NULL	49 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypertension is prevalent in 49 % of renal transplant recipients .
	manualset3
212068	3	419470	7	NULL	NULL	0	NULL	renal transplant recipients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypertension is prevalent in 49 % of renal transplant recipients .
	manualset3
212069	1	419471	7	NULL	NULL	0	NULL	 controlled volunteer studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Later , carefully controlled volunteer studies did not confirm the existence of the specific key symptoms , although one study of self-reported sensitive ( SRS ) people did suggest that a threshold at about 11-15 % MTBE in gasoline may exist for SRSs in total symptom scores .
	manualset3
212070	2	419471	7	NULL	NULL	0	NULL	existence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Later , carefully controlled volunteer studies did not confirm the existence of the specific key symptoms , although one study of self-reported sensitive ( SRS ) people did suggest that a threshold at about 11-15 % MTBE in gasoline may exist for SRSs in total symptom scores .
	manualset3
212071	3	419471	7	NULL	NULL	0	NULL	specific key symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Later , carefully controlled volunteer studies did not confirm the existence of the specific key symptoms , although one study of self-reported sensitive ( SRS ) people did suggest that a threshold at about 11-15 % MTBE in gasoline may exist for SRSs in total symptom scores .
	manualset3
212072	4	419471	7	NULL	NULL	0	NULL	one study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Later , carefully controlled volunteer studies did not confirm the existence of the specific key symptoms , although one study of self-reported sensitive ( SRS ) people did suggest that a threshold at about 11-15 % MTBE in gasoline may exist for SRSs in total symptom scores .
	manualset3
212073	5	419471	7	NULL	NULL	0	NULL	self-reported sensitive ( SRS ) people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Later , carefully controlled volunteer studies did not confirm the existence of the specific key symptoms , although one study of self-reported sensitive ( SRS ) people did suggest that a threshold at about 11-15 % MTBE in gasoline may exist for SRSs in total symptom scores .
	manualset3
212074	6	419471	7	NULL	NULL	0	NULL	threshold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Later , carefully controlled volunteer studies did not confirm the existence of the specific key symptoms , although one study of self-reported sensitive ( SRS ) people did suggest that a threshold at about 11-15 % MTBE in gasoline may exist for SRSs in total symptom scores .
	manualset3
212075	7	419471	7	NULL	NULL	0	NULL	11-15 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Later , carefully controlled volunteer studies did not confirm the existence of the specific key symptoms , although one study of self-reported sensitive ( SRS ) people did suggest that a threshold at about 11-15 % MTBE in gasoline may exist for SRSs in total symptom scores .
	manualset3
212076	8	419471	7	NULL	NULL	0	NULL	MTBE	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Later , carefully controlled volunteer studies did not confirm the existence of the specific key symptoms , although one study of self-reported sensitive ( SRS ) people did suggest that a threshold at about 11-15 % MTBE in gasoline may exist for SRSs in total symptom scores .
	manualset3
212077	9	419471	7	NULL	NULL	0	NULL	gasoline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Later , carefully controlled volunteer studies did not confirm the existence of the specific key symptoms , although one study of self-reported sensitive ( SRS ) people did suggest that a threshold at about 11-15 % MTBE in gasoline may exist for SRSs in total symptom scores .
	manualset3
212078	10	419471	7	NULL	NULL	0	NULL	SRSs	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Later , carefully controlled volunteer studies did not confirm the existence of the specific key symptoms , although one study of self-reported sensitive ( SRS ) people did suggest that a threshold at about 11-15 % MTBE in gasoline may exist for SRSs in total symptom scores .
	manualset3
212079	11	419471	7	NULL	NULL	0	NULL	total symptom scores	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Later , carefully controlled volunteer studies did not confirm the existence of the specific key symptoms , although one study of self-reported sensitive ( SRS ) people did suggest that a threshold at about 11-15 % MTBE in gasoline may exist for SRSs in total symptom scores .
	manualset3
212162	1	419472	7	NULL	NULL	0	NULL	glucose feeding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , glucose feeding with IMI plus adrenaline or insulin in these animals did not result in any significant alteration in blood glucose level ( BGL ) , as compared to oral glucose plus single doses of adrenaline or insulin .
	manualset3
212163	2	419472	7	NULL	NULL	0	NULL	IMI plus adrenaline 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , glucose feeding with IMI plus adrenaline or insulin in these animals did not result in any significant alteration in blood glucose level ( BGL ) , as compared to oral glucose plus single doses of adrenaline or insulin .
	manualset3
212164	3	419472	7	NULL	NULL	0	NULL	IMI plus insulin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , glucose feeding with IMI plus adrenaline or insulin in these animals did not result in any significant alteration in blood glucose level ( BGL ) , as compared to oral glucose plus single doses of adrenaline or insulin .
	manualset3
212165	4	419472	7	NULL	NULL	0	NULL	 animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , glucose feeding with IMI plus adrenaline or insulin in these animals did not result in any significant alteration in blood glucose level ( BGL ) , as compared to oral glucose plus single doses of adrenaline or insulin .
	manualset3
212166	5	419472	7	NULL	NULL	0	NULL	alteration 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , glucose feeding with IMI plus adrenaline or insulin in these animals did not result in any significant alteration in blood glucose level ( BGL ) , as compared to oral glucose plus single doses of adrenaline or insulin .
	manualset3
212167	6	419472	7	NULL	NULL	0	NULL	blood glucose level ( BGL ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , glucose feeding with IMI plus adrenaline or insulin in these animals did not result in any significant alteration in blood glucose level ( BGL ) , as compared to oral glucose plus single doses of adrenaline or insulin .
	manualset3
212168	7	419472	7	NULL	NULL	0	NULL	 oral glucose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , glucose feeding with IMI plus adrenaline or insulin in these animals did not result in any significant alteration in blood glucose level ( BGL ) , as compared to oral glucose plus single doses of adrenaline or insulin .
	manualset3
212169	8	419472	7	NULL	NULL	0	NULL	single doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , glucose feeding with IMI plus adrenaline or insulin in these animals did not result in any significant alteration in blood glucose level ( BGL ) , as compared to oral glucose plus single doses of adrenaline or insulin .
	manualset3
212170	9	419472	7	NULL	NULL	0	NULL	adrenaline 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , glucose feeding with IMI plus adrenaline or insulin in these animals did not result in any significant alteration in blood glucose level ( BGL ) , as compared to oral glucose plus single doses of adrenaline or insulin .
	manualset3
212171	10	419472	7	NULL	NULL	0	NULL	insulin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , glucose feeding with IMI plus adrenaline or insulin in these animals did not result in any significant alteration in blood glucose level ( BGL ) , as compared to oral glucose plus single doses of adrenaline or insulin .
	manualset3
212172	1	419473	7	NULL	NULL	0	NULL	Very long-chain polyunsaturated fatty acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Very long-chain polyunsaturated fatty acids are the major acyl groups of sphingomyelins and ceramides in the head of mammalian spermatozoa .
	manualset3
212173	2	419473	7	NULL	NULL	0	NULL	major acyl groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Very long-chain polyunsaturated fatty acids are the major acyl groups of sphingomyelins and ceramides in the head of mammalian spermatozoa .
	manualset3
212174	3	419473	7	NULL	NULL	0	NULL	sphingomyelins	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Very long-chain polyunsaturated fatty acids are the major acyl groups of sphingomyelins and ceramides in the head of mammalian spermatozoa .
	manualset3
212175	4	419473	7	NULL	NULL	0	NULL	ceramides 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Very long-chain polyunsaturated fatty acids are the major acyl groups of sphingomyelins and ceramides in the head of mammalian spermatozoa .
	manualset3
212176	5	419473	7	NULL	NULL	NULL	NULL	head	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Very long-chain polyunsaturated fatty acids are the major acyl groups of sphingomyelins and ceramides in the head of mammalian spermatozoa .
	manualset3
212177	6	419473	7	NULL	NULL	NULL	NULL	mammalian spermatozoa	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Very long-chain polyunsaturated fatty acids are the major acyl groups of sphingomyelins and ceramides in the head of mammalian spermatozoa .
	manualset3
212178	1	419474	7	NULL	NULL	0	NULL	Para-aminobenzoic acid therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Para-aminobenzoic acid therapy in lymphoblastoma cutis and mycosis fungoides .
	manualset3
212179	2	419474	7	NULL	NULL	0	NULL	lymphoblastoma cutis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Para-aminobenzoic acid therapy in lymphoblastoma cutis and mycosis fungoides .
	manualset3
212180	3	419474	7	NULL	NULL	0	NULL	mycosis fungoides	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Para-aminobenzoic acid therapy in lymphoblastoma cutis and mycosis fungoides .
	manualset3
212181	1	419475	7	NULL	NULL	0	NULL	two duties	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When these two duties conflict , the latter obligation to the individual takes priority .
	manualset3
212182	2	419475	7	NULL	NULL	0	NULL	obligation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When these two duties conflict , the latter obligation to the individual takes priority .
	manualset3
212183	3	419475	7	NULL	NULL	0	NULL	 individual	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	When these two duties conflict , the latter obligation to the individual takes priority .
	manualset3
212184	1	419476	7	NULL	NULL	0	NULL	GH response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The GH response ( area under the curve + / - SE ) to IHG was significantly reduced by a concomitant ivt glucose infusion ( control , 1.0 + / - 0.1 ; IHG , 12.1 + / - 3.3 ; IHG plus ivt glucose , 7.0 + / - 1.2 microgram/L .120 min ) .
	manualset3
212185	2	419476	7	NULL	NULL	0	NULL	area under the curve + / - SE 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The GH response ( area under the curve + / - SE ) to IHG was significantly reduced by a concomitant ivt glucose infusion ( control , 1.0 + / - 0.1 ; IHG , 12.1 + / - 3.3 ; IHG plus ivt glucose , 7.0 + / - 1.2 microgram/L .120 min ) .
	manualset3
212186	3	419476	7	NULL	NULL	0	NULL	 IHG	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The GH response ( area under the curve + / - SE ) to IHG was significantly reduced by a concomitant ivt glucose infusion ( control , 1.0 + / - 0.1 ; IHG , 12.1 + / - 3.3 ; IHG plus ivt glucose , 7.0 + / - 1.2 microgram/L .120 min ) .
	manualset3
212187	4	419476	7	NULL	NULL	0	NULL	ivt glucose infusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The GH response ( area under the curve + / - SE ) to IHG was significantly reduced by a concomitant ivt glucose infusion ( control , 1.0 + / - 0.1 ; IHG , 12.1 + / - 3.3 ; IHG plus ivt glucose , 7.0 + / - 1.2 microgram/L .120 min ) .
	manualset3
212188	5	419476	7	NULL	NULL	NULL	NULL	control 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The GH response ( area under the curve + / - SE ) to IHG was significantly reduced by a concomitant ivt glucose infusion ( control , 1.0 + / - 0.1 ; IHG , 12.1 + / - 3.3 ; IHG plus ivt glucose , 7.0 + / - 1.2 microgram/L .120 min ) .
	manualset3
212189	7	419476	7	NULL	NULL	NULL	NULL	IHG 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The GH response ( area under the curve + / - SE ) to IHG was significantly reduced by a concomitant ivt glucose infusion ( control , 1.0 + / - 0.1 ; IHG , 12.1 + / - 3.3 ; IHG plus ivt glucose , 7.0 + / - 1.2 microgram/L .120 min ) .
	manualset3
212190	6	419476	7	NULL	NULL	0	NULL	1.0 + / - 0.1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The GH response ( area under the curve + / - SE ) to IHG was significantly reduced by a concomitant ivt glucose infusion ( control , 1.0 + / - 0.1 ; IHG , 12.1 + / - 3.3 ; IHG plus ivt glucose , 7.0 + / - 1.2 microgram/L .120 min ) .
	manualset3
212191	8	419476	7	NULL	NULL	0	NULL	12.1 + / - 3.3 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The GH response ( area under the curve + / - SE ) to IHG was significantly reduced by a concomitant ivt glucose infusion ( control , 1.0 + / - 0.1 ; IHG , 12.1 + / - 3.3 ; IHG plus ivt glucose , 7.0 + / - 1.2 microgram/L .120 min ) .
	manualset3
212192	9	419476	7	NULL	NULL	0	NULL	 IHG	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The GH response ( area under the curve + / - SE ) to IHG was significantly reduced by a concomitant ivt glucose infusion ( control , 1.0 + / - 0.1 ; IHG , 12.1 + / - 3.3 ; IHG plus ivt glucose , 7.0 + / - 1.2 microgram/L .120 min ) .
	manualset3
212193	10	419476	7	NULL	NULL	0	NULL	 ivt glucose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The GH response ( area under the curve + / - SE ) to IHG was significantly reduced by a concomitant ivt glucose infusion ( control , 1.0 + / - 0.1 ; IHG , 12.1 + / - 3.3 ; IHG plus ivt glucose , 7.0 + / - 1.2 microgram/L .120 min ) .
	manualset3
212194	11	419476	7	NULL	NULL	0	NULL	7.0 + / - 1.2 microgram/L .120 min	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The GH response ( area under the curve + / - SE ) to IHG was significantly reduced by a concomitant ivt glucose infusion ( control , 1.0 + / - 0.1 ; IHG , 12.1 + / - 3.3 ; IHG plus ivt glucose , 7.0 + / - 1.2 microgram/L .120 min ) .
	manualset3
212195	1	419477	7	NULL	NULL	0	NULL	Cytostatic therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cytostatic therapy in lung tumors ) .
	manualset3
212196	2	419477	7	NULL	NULL	0	NULL	lung tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cytostatic therapy in lung tumors ) .
	manualset3
212197	1	419478	7	NULL	NULL	0	NULL	mast cell disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Although mast cell disease is most commonly identified in the skin , involvement of the skeletal , hematopoietic , gastrointestinal , cardiopulmonary , and central nervous systems may be seen .
	manualset3
212198	2	419478	7	NULL	NULL	0	NULL	 skin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although mast cell disease is most commonly identified in the skin , involvement of the skeletal , hematopoietic , gastrointestinal , cardiopulmonary , and central nervous systems may be seen .
	manualset3
212199	3	419478	7	NULL	NULL	0	NULL	skeletal system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although mast cell disease is most commonly identified in the skin , involvement of the skeletal , hematopoietic , gastrointestinal , cardiopulmonary , and central nervous systems may be seen .
	manualset3
212200	4	419478	7	NULL	NULL	0	NULL	hematopoietic system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although mast cell disease is most commonly identified in the skin , involvement of the skeletal , hematopoietic , gastrointestinal , cardiopulmonary , and central nervous systems may be seen .
	manualset3
212201	5	419478	7	NULL	NULL	0	NULL	gastrointestinal system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although mast cell disease is most commonly identified in the skin , involvement of the skeletal , hematopoietic , gastrointestinal , cardiopulmonary , and central nervous systems may be seen .
	manualset3
212202	6	419478	7	NULL	NULL	0	NULL	cardiopulmonary system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although mast cell disease is most commonly identified in the skin , involvement of the skeletal , hematopoietic , gastrointestinal , cardiopulmonary , and central nervous systems may be seen .
	manualset3
212203	7	419478	7	NULL	NULL	0	NULL	central nervous systems	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although mast cell disease is most commonly identified in the skin , involvement of the skeletal , hematopoietic , gastrointestinal , cardiopulmonary , and central nervous systems may be seen .
	manualset3
212204	1	419479	7	NULL	NULL	0	NULL	13 factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the 13 factors examined which might be responsible for inducing NEC , only 2 were correlated with G-I disorders : low birth weight ( less than 1 , 500 gm ) and occurrence of secondary apnea or asphyxia incidents during mechanical ventilation .
	manualset3
212205	2	419479	7	NULL	NULL	0	NULL	NEC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the 13 factors examined which might be responsible for inducing NEC , only 2 were correlated with G-I disorders : low birth weight ( less than 1 , 500 gm ) and occurrence of secondary apnea or asphyxia incidents during mechanical ventilation .
	manualset3
212206	3	419479	7	NULL	NULL	0	NULL	 2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the 13 factors examined which might be responsible for inducing NEC , only 2 were correlated with G-I disorders : low birth weight ( less than 1 , 500 gm ) and occurrence of secondary apnea or asphyxia incidents during mechanical ventilation .
	manualset3
212207	4	419479	7	NULL	NULL	0	NULL	G-I disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the 13 factors examined which might be responsible for inducing NEC , only 2 were correlated with G-I disorders : low birth weight ( less than 1 , 500 gm ) and occurrence of secondary apnea or asphyxia incidents during mechanical ventilation .
	manualset3
212208	5	419479	7	NULL	NULL	0	NULL	low birth weight	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the 13 factors examined which might be responsible for inducing NEC , only 2 were correlated with G-I disorders : low birth weight ( less than 1 , 500 gm ) and occurrence of secondary apnea or asphyxia incidents during mechanical ventilation .
	manualset3
212209	6	419479	7	NULL	NULL	0	NULL	1 , 500 gm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the 13 factors examined which might be responsible for inducing NEC , only 2 were correlated with G-I disorders : low birth weight ( less than 1 , 500 gm ) and occurrence of secondary apnea or asphyxia incidents during mechanical ventilation .
	manualset3
212210	7	419479	7	NULL	NULL	0	NULL	occurrence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the 13 factors examined which might be responsible for inducing NEC , only 2 were correlated with G-I disorders : low birth weight ( less than 1 , 500 gm ) and occurrence of secondary apnea or asphyxia incidents during mechanical ventilation .
	manualset3
212211	8	419479	7	NULL	NULL	0	NULL	secondary apnea	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the 13 factors examined which might be responsible for inducing NEC , only 2 were correlated with G-I disorders : low birth weight ( less than 1 , 500 gm ) and occurrence of secondary apnea or asphyxia incidents during mechanical ventilation .
	manualset3
212212	9	419479	7	NULL	NULL	0	NULL	asphyxia incidents	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the 13 factors examined which might be responsible for inducing NEC , only 2 were correlated with G-I disorders : low birth weight ( less than 1 , 500 gm ) and occurrence of secondary apnea or asphyxia incidents during mechanical ventilation .
	manualset3
212213	10	419479	7	NULL	NULL	0	NULL	mechanical ventilation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the 13 factors examined which might be responsible for inducing NEC , only 2 were correlated with G-I disorders : low birth weight ( less than 1 , 500 gm ) and occurrence of secondary apnea or asphyxia incidents during mechanical ventilation .
	manualset3
212214	1	419480	7	NULL	NULL	0	NULL	Amphibian chytridiomycosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Amphibian chytridiomycosis is an infectious disease caused by the fungus Batrachochytrium dendrobatidis ( Bd ) that is implicated in the worldwide decline and extinction of amphibians .
	manualset3
212215	2	419480	7	NULL	NULL	0	NULL	infectious disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Amphibian chytridiomycosis is an infectious disease caused by the fungus Batrachochytrium dendrobatidis ( Bd ) that is implicated in the worldwide decline and extinction of amphibians .
	manualset3
212216	3	419480	7	NULL	NULL	0	NULL	fungus Batrachochytrium dendrobatidis ( Bd )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Amphibian chytridiomycosis is an infectious disease caused by the fungus Batrachochytrium dendrobatidis ( Bd ) that is implicated in the worldwide decline and extinction of amphibians .
	manualset3
212217	4	419480	7	NULL	NULL	0	NULL	worldwide	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Amphibian chytridiomycosis is an infectious disease caused by the fungus Batrachochytrium dendrobatidis ( Bd ) that is implicated in the worldwide decline and extinction of amphibians .
	manualset3
212218	5	419480	7	NULL	NULL	0	NULL	extinction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Amphibian chytridiomycosis is an infectious disease caused by the fungus Batrachochytrium dendrobatidis ( Bd ) that is implicated in the worldwide decline and extinction of amphibians .
	manualset3
212219	6	419480	7	NULL	NULL	0	NULL	amphibians	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Amphibian chytridiomycosis is an infectious disease caused by the fungus Batrachochytrium dendrobatidis ( Bd ) that is implicated in the worldwide decline and extinction of amphibians .
	manualset3
212220	1	419481	7	NULL	NULL	0	NULL	Histopathological studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Histopathological studies on the nature of lymph node tuberculosis .
	manualset3
212221	2	419481	7	NULL	NULL	0	NULL	 nature	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histopathological studies on the nature of lymph node tuberculosis .
	manualset3
212222	3	419481	7	NULL	NULL	0	NULL	lymph node tuberculosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Histopathological studies on the nature of lymph node tuberculosis .
	manualset3
212223	1	419482	7	NULL	NULL	0	NULL	Peripheral plasma concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral plasma or serum concentrations of haptoglobin , seromucoid , ceruloplasmin and 15-keto-13 , 14 - dihydro-prostaglandin F2 alpha ( PGFM ) were measured up to six weeks postpartum .
	manualset3
212224	2	419482	7	NULL	NULL	0	NULL	serum concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral plasma or serum concentrations of haptoglobin , seromucoid , ceruloplasmin and 15-keto-13 , 14 - dihydro-prostaglandin F2 alpha ( PGFM ) were measured up to six weeks postpartum .
	manualset3
212225	3	419482	7	NULL	NULL	0	NULL	haptoglobin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral plasma or serum concentrations of haptoglobin , seromucoid , ceruloplasmin and 15-keto-13 , 14 - dihydro-prostaglandin F2 alpha ( PGFM ) were measured up to six weeks postpartum .
	manualset3
212226	4	419482	7	NULL	NULL	0	NULL	seromucoid	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral plasma or serum concentrations of haptoglobin , seromucoid , ceruloplasmin and 15-keto-13 , 14 - dihydro-prostaglandin F2 alpha ( PGFM ) were measured up to six weeks postpartum .
	manualset3
212227	5	419482	7	NULL	NULL	0	NULL	ceruloplasmin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral plasma or serum concentrations of haptoglobin , seromucoid , ceruloplasmin and 15-keto-13 , 14 - dihydro-prostaglandin F2 alpha ( PGFM ) were measured up to six weeks postpartum .
	manualset3
212228	6	419482	7	NULL	NULL	0	NULL	15-keto-13 , 14 - dihydro-prostaglandin F2 alpha ( PGFM )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral plasma or serum concentrations of haptoglobin , seromucoid , ceruloplasmin and 15-keto-13 , 14 - dihydro-prostaglandin F2 alpha ( PGFM ) were measured up to six weeks postpartum .
	manualset3
212229	7	419482	7	NULL	NULL	0	NULL	six weeks postpartum	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Peripheral plasma or serum concentrations of haptoglobin , seromucoid , ceruloplasmin and 15-keto-13 , 14 - dihydro-prostaglandin F2 alpha ( PGFM ) were measured up to six weeks postpartum .
	manualset3
212230	1	419483	7	NULL	NULL	0	NULL	MINK	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	MINK encodes a 1300 amino acid polypeptide , consisting of an N-terminal kinase domain , a proline-rich intermediate region , and a C-terminal GCK homology region .
	manualset3
212231	2	419483	7	NULL	NULL	0	NULL	1300 amino acid polypeptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	MINK encodes a 1300 amino acid polypeptide , consisting of an N-terminal kinase domain , a proline-rich intermediate region , and a C-terminal GCK homology region .
	manualset3
212232	3	419483	7	NULL	NULL	0	NULL	N-terminal kinase domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	MINK encodes a 1300 amino acid polypeptide , consisting of an N-terminal kinase domain , a proline-rich intermediate region , and a C-terminal GCK homology region .
	manualset3
212233	4	419483	7	NULL	NULL	0	NULL	proline-rich intermediate region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	MINK encodes a 1300 amino acid polypeptide , consisting of an N-terminal kinase domain , a proline-rich intermediate region , and a C-terminal GCK homology region .
	manualset3
212234	5	419483	7	NULL	NULL	0	NULL	C-terminal GCK homology region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	MINK encodes a 1300 amino acid polypeptide , consisting of an N-terminal kinase domain , a proline-rich intermediate region , and a C-terminal GCK homology region .
	manualset3
212235	1	419484	7	NULL	NULL	0	NULL	Recording	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recording of chick embryo movements and their correlation with joint development .
	manualset3
212236	2	419484	7	NULL	NULL	0	NULL	chick embryo movements	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recording of chick embryo movements and their correlation with joint development .
	manualset3
212237	3	419484	7	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Recording of chick embryo movements and their correlation with joint development .
	manualset3
212238	4	419484	7	NULL	NULL	0	NULL	joint development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recording of chick embryo movements and their correlation with joint development .
	manualset3
212239	1	419485	7	NULL	NULL	0	NULL	stress	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Given high consequences , stress is presumed to reach its maximum when demand is substantially greater than ability ( overload ) or when ability is substantially greater than demand ( underload ) .
	manualset3
212240	2	419485	7	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Given high consequences , stress is presumed to reach its maximum when demand is substantially greater than ability ( overload ) or when ability is substantially greater than demand ( underload ) .
	manualset3
212241	3	419485	7	NULL	NULL	0	NULL	overload	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Given high consequences , stress is presumed to reach its maximum when demand is substantially greater than ability ( overload ) or when ability is substantially greater than demand ( underload ) .
	manualset3
212242	4	419485	7	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Given high consequences , stress is presumed to reach its maximum when demand is substantially greater than ability ( overload ) or when ability is substantially greater than demand ( underload ) .
	manualset3
212243	5	419485	7	NULL	NULL	0	NULL	underload	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Given high consequences , stress is presumed to reach its maximum when demand is substantially greater than ability ( overload ) or when ability is substantially greater than demand ( underload ) .
	manualset3
212244	6	419485	7	NULL	NULL	0	NULL	 high consequences	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Given high consequences , stress is presumed to reach its maximum when demand is substantially greater than ability ( overload ) or when ability is substantially greater than demand ( underload ) .
	manualset3
212245	7	419485	7	NULL	NULL	0	NULL	demand	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Given high consequences , stress is presumed to reach its maximum when demand is substantially greater than ability ( overload ) or when ability is substantially greater than demand ( underload ) .
	manualset3
215149	8	419485	7	NULL	NULL	0	NULL	maximum	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Given high consequences , stress is presumed to reach its maximum when demand is substantially greater than ability ( overload ) or when ability is substantially greater than demand ( underload ) .
	manualset3
212246	1	419486	7	NULL	NULL	0	NULL	mineralocorticoid	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although mineralocorticoid and mineralocorticoid receptor ( MR ) have attracted increasing attention in the field of vascular injury , including the heart , kidney , and vessels , little is known about the role of mineralocorticoid in PF .
	manualset3
212247	2	419486	7	NULL	NULL	0	NULL	mineralocorticoid receptor ( MR )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although mineralocorticoid and mineralocorticoid receptor ( MR ) have attracted increasing attention in the field of vascular injury , including the heart , kidney , and vessels , little is known about the role of mineralocorticoid in PF .
	manualset3
212248	3	419486	7	NULL	NULL	0	NULL	 increasing attention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although mineralocorticoid and mineralocorticoid receptor ( MR ) have attracted increasing attention in the field of vascular injury , including the heart , kidney , and vessels , little is known about the role of mineralocorticoid in PF .
	manualset3
212249	4	419486	7	NULL	NULL	0	NULL	field	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Although mineralocorticoid and mineralocorticoid receptor ( MR ) have attracted increasing attention in the field of vascular injury , including the heart , kidney , and vessels , little is known about the role of mineralocorticoid in PF .
	manualset3
212250	5	419486	7	NULL	NULL	0	NULL	vascular injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although mineralocorticoid and mineralocorticoid receptor ( MR ) have attracted increasing attention in the field of vascular injury , including the heart , kidney , and vessels , little is known about the role of mineralocorticoid in PF .
	manualset3
212251	6	419486	7	NULL	NULL	0	NULL	heart	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although mineralocorticoid and mineralocorticoid receptor ( MR ) have attracted increasing attention in the field of vascular injury , including the heart , kidney , and vessels , little is known about the role of mineralocorticoid in PF .
	manualset3
212252	7	419486	7	NULL	NULL	0	NULL	 kidney	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although mineralocorticoid and mineralocorticoid receptor ( MR ) have attracted increasing attention in the field of vascular injury , including the heart , kidney , and vessels , little is known about the role of mineralocorticoid in PF .
	manualset3
212253	8	419486	7	NULL	NULL	0	NULL	vessels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although mineralocorticoid and mineralocorticoid receptor ( MR ) have attracted increasing attention in the field of vascular injury , including the heart , kidney , and vessels , little is known about the role of mineralocorticoid in PF .
	manualset3
212254	9	419486	7	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although mineralocorticoid and mineralocorticoid receptor ( MR ) have attracted increasing attention in the field of vascular injury , including the heart , kidney , and vessels , little is known about the role of mineralocorticoid in PF .
	manualset3
212255	10	419486	7	NULL	NULL	0	NULL	mineralocorticoid	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although mineralocorticoid and mineralocorticoid receptor ( MR ) have attracted increasing attention in the field of vascular injury , including the heart , kidney , and vessels , little is known about the role of mineralocorticoid in PF .
	manualset3
212256	11	419486	7	NULL	NULL	0	NULL	PF	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Although mineralocorticoid and mineralocorticoid receptor ( MR ) have attracted increasing attention in the field of vascular injury , including the heart , kidney , and vessels , little is known about the role of mineralocorticoid in PF .
	manualset3
212257	1	419487	7	NULL	NULL	0	NULL	r-SAT treated rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The r-SAT treated rats lost more body weight than saline treated animals the first day after treatment .
	manualset3
212258	2	419487	7	NULL	NULL	0	NULL	body weight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The r-SAT treated rats lost more body weight than saline treated animals the first day after treatment .
	manualset3
212259	3	419487	7	NULL	NULL	0	NULL	saline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The r-SAT treated rats lost more body weight than saline treated animals the first day after treatment .
	manualset3
212260	4	419487	7	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The r-SAT treated rats lost more body weight than saline treated animals the first day after treatment .
	manualset3
212261	5	419487	7	NULL	NULL	NULL	NULL	first day	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The r-SAT treated rats lost more body weight than saline treated animals the first day after treatment .
	manualset3
212262	6	419487	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The r-SAT treated rats lost more body weight than saline treated animals the first day after treatment .
	manualset3
212263	1	419488	7	NULL	NULL	0	NULL	Removal of the suture	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of the suture led to a triphasic restitution of blood flow consisting of a fast initial rise , a secondary decline , and final normalization .
	manualset3
212264	2	419488	7	NULL	NULL	0	NULL	triphasic restitution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of the suture led to a triphasic restitution of blood flow consisting of a fast initial rise , a secondary decline , and final normalization .
	manualset3
212265	3	419488	7	NULL	NULL	0	NULL	 blood flow 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of the suture led to a triphasic restitution of blood flow consisting of a fast initial rise , a secondary decline , and final normalization .
	manualset3
212266	4	419488	7	NULL	NULL	0	NULL	fast initial rise	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of the suture led to a triphasic restitution of blood flow consisting of a fast initial rise , a secondary decline , and final normalization .
	manualset3
212267	5	419488	7	NULL	NULL	NULL	NULL	secondary decline	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Removal of the suture led to a triphasic restitution of blood flow consisting of a fast initial rise , a secondary decline , and final normalization .
	manualset3
212268	6	419488	7	NULL	NULL	0	NULL	final normalization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Removal of the suture led to a triphasic restitution of blood flow consisting of a fast initial rise , a secondary decline , and final normalization .
	manualset3
212269	1	419489	7	NULL	NULL	NULL	NULL	BCG immunization coverage	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BCG immunization coverage was high ( 85 % ) , but measles immunization coverage was moderate ( 48 % ) .
	manualset3
212270	2	419489	7	NULL	NULL	0	NULL	85 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	BCG immunization coverage was high ( 85 % ) , but measles immunization coverage was moderate ( 48 % ) .
	manualset3
212271	3	419489	7	NULL	NULL	0	NULL	measles immunization coverage	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	BCG immunization coverage was high ( 85 % ) , but measles immunization coverage was moderate ( 48 % ) .
	manualset3
212272	4	419489	7	NULL	NULL	0	NULL	48 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	BCG immunization coverage was high ( 85 % ) , but measles immunization coverage was moderate ( 48 % ) .
	manualset3
212273	1	419490	7	NULL	NULL	0	NULL	78-year-old man	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A 78-year-old man , previously treated for prostate and colorectal cancer , was admitted to the hospital because of persistent fever .
	manualset3
212274	2	419490	7	NULL	NULL	0	NULL	prostate cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A 78-year-old man , previously treated for prostate and colorectal cancer , was admitted to the hospital because of persistent fever .
	manualset3
212275	3	419490	7	NULL	NULL	0	NULL	colorectal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A 78-year-old man , previously treated for prostate and colorectal cancer , was admitted to the hospital because of persistent fever .
	manualset3
212276	4	419490	7	NULL	NULL	0	NULL	hospital	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A 78-year-old man , previously treated for prostate and colorectal cancer , was admitted to the hospital because of persistent fever .
	manualset3
212277	5	419490	7	NULL	NULL	0	NULL	persistent fever	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A 78-year-old man , previously treated for prostate and colorectal cancer , was admitted to the hospital because of persistent fever .
	manualset3
212278	1	419491	7	NULL	NULL	0	NULL	report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report , we used COS-7 cells transfected with the dopamine D1 receptor ( D1R ) to illustrate the signaling mechanism for Gs-mediated JNK activation .
	manualset3
212279	2	419491	7	NULL	NULL	0	NULL	COS-7 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report , we used COS-7 cells transfected with the dopamine D1 receptor ( D1R ) to illustrate the signaling mechanism for Gs-mediated JNK activation .
	manualset3
212280	3	419491	7	NULL	NULL	0	NULL	dopamine D1 receptor ( D1R )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report , we used COS-7 cells transfected with the dopamine D1 receptor ( D1R ) to illustrate the signaling mechanism for Gs-mediated JNK activation .
	manualset3
212281	4	419491	7	NULL	NULL	0	NULL	signaling mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report , we used COS-7 cells transfected with the dopamine D1 receptor ( D1R ) to illustrate the signaling mechanism for Gs-mediated JNK activation .
	manualset3
212282	5	419491	7	NULL	NULL	0	NULL	Gs-mediated JNK activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this report , we used COS-7 cells transfected with the dopamine D1 receptor ( D1R ) to illustrate the signaling mechanism for Gs-mediated JNK activation .
	manualset3
212283	1	419492	7	NULL	NULL	0	NULL	Evidence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence derived by the process of elimination indicates that the spontaneous call depends on the concerted action of a continuous band of rostral limbic cortex comprising parts of areas 24 , 25 , and 12 .
	manualset3
212284	2	419492	7	NULL	NULL	0	NULL	process of elimination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence derived by the process of elimination indicates that the spontaneous call depends on the concerted action of a continuous band of rostral limbic cortex comprising parts of areas 24 , 25 , and 12 .
	manualset3
212285	3	419492	7	NULL	NULL	0	NULL	spontaneous call	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence derived by the process of elimination indicates that the spontaneous call depends on the concerted action of a continuous band of rostral limbic cortex comprising parts of areas 24 , 25 , and 12 .
	manualset3
212286	4	419492	7	NULL	NULL	0	NULL	concerted action	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence derived by the process of elimination indicates that the spontaneous call depends on the concerted action of a continuous band of rostral limbic cortex comprising parts of areas 24 , 25 , and 12 .
	manualset3
212287	5	419492	7	NULL	NULL	0	NULL	continuous band	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence derived by the process of elimination indicates that the spontaneous call depends on the concerted action of a continuous band of rostral limbic cortex comprising parts of areas 24 , 25 , and 12 .
	manualset3
212288	6	419492	7	NULL	NULL	0	NULL	rostral limbic cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence derived by the process of elimination indicates that the spontaneous call depends on the concerted action of a continuous band of rostral limbic cortex comprising parts of areas 24 , 25 , and 12 .
	manualset3
212289	7	419492	7	NULL	NULL	0	NULL	parts of areas 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence derived by the process of elimination indicates that the spontaneous call depends on the concerted action of a continuous band of rostral limbic cortex comprising parts of areas 24 , 25 , and 12 .
	manualset3
212290	8	419492	7	NULL	NULL	0	NULL	24	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence derived by the process of elimination indicates that the spontaneous call depends on the concerted action of a continuous band of rostral limbic cortex comprising parts of areas 24 , 25 , and 12 .
	manualset3
212291	9	419492	7	NULL	NULL	0	NULL	25	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence derived by the process of elimination indicates that the spontaneous call depends on the concerted action of a continuous band of rostral limbic cortex comprising parts of areas 24 , 25 , and 12 .
	manualset3
212292	10	419492	7	NULL	NULL	0	NULL	12	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence derived by the process of elimination indicates that the spontaneous call depends on the concerted action of a continuous band of rostral limbic cortex comprising parts of areas 24 , 25 , and 12 .
	manualset3
212293	1	419493	7	NULL	NULL	0	NULL	Concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentration of selenium in whole blood and plasma , lipid peroxides in plasma , and glutathione peroxidase activities in red blood cell hemolysates and plasma were determined in 49 coal power plant workers and in 50 rubber factory workers .
	manualset3
212294	2	419493	7	NULL	NULL	0	NULL	selenium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentration of selenium in whole blood and plasma , lipid peroxides in plasma , and glutathione peroxidase activities in red blood cell hemolysates and plasma were determined in 49 coal power plant workers and in 50 rubber factory workers .
	manualset3
212295	3	419493	7	NULL	NULL	0	NULL	whole blood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentration of selenium in whole blood and plasma , lipid peroxides in plasma , and glutathione peroxidase activities in red blood cell hemolysates and plasma were determined in 49 coal power plant workers and in 50 rubber factory workers .
	manualset3
212296	4	419493	7	NULL	NULL	0	NULL	plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentration of selenium in whole blood and plasma , lipid peroxides in plasma , and glutathione peroxidase activities in red blood cell hemolysates and plasma were determined in 49 coal power plant workers and in 50 rubber factory workers .
	manualset3
212297	5	419493	7	NULL	NULL	0	NULL	 lipid peroxides 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentration of selenium in whole blood and plasma , lipid peroxides in plasma , and glutathione peroxidase activities in red blood cell hemolysates and plasma were determined in 49 coal power plant workers and in 50 rubber factory workers .
	manualset3
212298	6	419493	7	NULL	NULL	0	NULL	plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentration of selenium in whole blood and plasma , lipid peroxides in plasma , and glutathione peroxidase activities in red blood cell hemolysates and plasma were determined in 49 coal power plant workers and in 50 rubber factory workers .
	manualset3
212299	7	419493	7	NULL	NULL	0	NULL	glutathione peroxidase activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentration of selenium in whole blood and plasma , lipid peroxides in plasma , and glutathione peroxidase activities in red blood cell hemolysates and plasma were determined in 49 coal power plant workers and in 50 rubber factory workers .
	manualset3
212300	8	419493	7	NULL	NULL	0	NULL	red blood cell hemolysates	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentration of selenium in whole blood and plasma , lipid peroxides in plasma , and glutathione peroxidase activities in red blood cell hemolysates and plasma were determined in 49 coal power plant workers and in 50 rubber factory workers .
	manualset3
212301	9	419493	7	NULL	NULL	0	NULL	plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentration of selenium in whole blood and plasma , lipid peroxides in plasma , and glutathione peroxidase activities in red blood cell hemolysates and plasma were determined in 49 coal power plant workers and in 50 rubber factory workers .
	manualset3
212302	10	419493	7	NULL	NULL	0	NULL	49 coal power plant workers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentration of selenium in whole blood and plasma , lipid peroxides in plasma , and glutathione peroxidase activities in red blood cell hemolysates and plasma were determined in 49 coal power plant workers and in 50 rubber factory workers .
	manualset3
212303	11	419493	7	NULL	NULL	0	NULL	50 rubber factory workers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentration of selenium in whole blood and plasma , lipid peroxides in plasma , and glutathione peroxidase activities in red blood cell hemolysates and plasma were determined in 49 coal power plant workers and in 50 rubber factory workers .
	manualset3
212304	1	419494	7	NULL	NULL	0	NULL	assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although more assays are required , these results show that IQMF-4 appears to be a potent analgesic compound with an interesting peripheral component , and reduced ability to induce dependence .
	manualset3
212305	2	419494	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although more assays are required , these results show that IQMF-4 appears to be a potent analgesic compound with an interesting peripheral component , and reduced ability to induce dependence .
	manualset3
212306	3	419494	7	NULL	NULL	0	NULL	IQMF-4	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although more assays are required , these results show that IQMF-4 appears to be a potent analgesic compound with an interesting peripheral component , and reduced ability to induce dependence .
	manualset3
212307	4	419494	7	NULL	NULL	0	NULL	analgesic compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although more assays are required , these results show that IQMF-4 appears to be a potent analgesic compound with an interesting peripheral component , and reduced ability to induce dependence .
	manualset3
212308	5	419494	7	NULL	NULL	0	NULL	peripheral component	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although more assays are required , these results show that IQMF-4 appears to be a potent analgesic compound with an interesting peripheral component , and reduced ability to induce dependence .
	manualset3
212309	6	419494	7	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although more assays are required , these results show that IQMF-4 appears to be a potent analgesic compound with an interesting peripheral component , and reduced ability to induce dependence .
	manualset3
212310	7	419494	7	NULL	NULL	0	NULL	dependence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although more assays are required , these results show that IQMF-4 appears to be a potent analgesic compound with an interesting peripheral component , and reduced ability to induce dependence .
	manualset3
212311	1	419495	7	NULL	NULL	NULL	NULL	Axios river basin	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The Axios river basin is an area of high agricultural importance for Macedonia , Northern Greece .
	manualset3
212312	2	419495	7	NULL	NULL	0	NULL	area	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The Axios river basin is an area of high agricultural importance for Macedonia , Northern Greece .
	manualset3
212313	3	419495	7	NULL	NULL	0	NULL	high agricultural importance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Axios river basin is an area of high agricultural importance for Macedonia , Northern Greece .
	manualset3
212314	4	419495	7	NULL	NULL	0	NULL	Macedonia	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The Axios river basin is an area of high agricultural importance for Macedonia , Northern Greece .
	manualset3
212315	5	419495	7	NULL	NULL	0	NULL	Northern Greece	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The Axios river basin is an area of high agricultural importance for Macedonia , Northern Greece .
	manualset3
212316	1	419496	7	NULL	NULL	0	NULL	DA neuron survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Excellent DA neuron survival , function and lack of neural overgrowth in the three animal models indicate promise for the development of cell-based therapies in Parkinson 's disease .
	manualset3
212317	2	419496	7	NULL	NULL	0	NULL	function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Excellent DA neuron survival , function and lack of neural overgrowth in the three animal models indicate promise for the development of cell-based therapies in Parkinson 's disease .
	manualset3
212318	3	419496	7	NULL	NULL	0	NULL	lack of neural overgrowth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Excellent DA neuron survival , function and lack of neural overgrowth in the three animal models indicate promise for the development of cell-based therapies in Parkinson 's disease .
	manualset3
212319	4	419496	7	NULL	NULL	0	NULL	three animal models	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Excellent DA neuron survival , function and lack of neural overgrowth in the three animal models indicate promise for the development of cell-based therapies in Parkinson 's disease .
	manualset3
212320	5	419496	7	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Excellent DA neuron survival , function and lack of neural overgrowth in the three animal models indicate promise for the development of cell-based therapies in Parkinson 's disease .
	manualset3
212321	6	419496	7	NULL	NULL	0	NULL	cell-based therapies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Excellent DA neuron survival , function and lack of neural overgrowth in the three animal models indicate promise for the development of cell-based therapies in Parkinson 's disease .
	manualset3
212322	7	419496	7	NULL	NULL	0	NULL	Parkinson 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Excellent DA neuron survival , function and lack of neural overgrowth in the three animal models indicate promise for the development of cell-based therapies in Parkinson 's disease .
	manualset3
212323	1	419497	7	NULL	NULL	0	NULL	competition assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a competition assay , fluid-phase flvWF appeared to inhibit efficiently the binding of Factor VIII to immobilized vWF isolated from plasma , whereas vWFdelpro did not influence Factor VIII binding .
	manualset3
212324	2	419497	7	NULL	NULL	0	NULL	fluid-phase flvWF	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a competition assay , fluid-phase flvWF appeared to inhibit efficiently the binding of Factor VIII to immobilized vWF isolated from plasma , whereas vWFdelpro did not influence Factor VIII binding .
	manualset3
212325	3	419497	7	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In a competition assay , fluid-phase flvWF appeared to inhibit efficiently the binding of Factor VIII to immobilized vWF isolated from plasma , whereas vWFdelpro did not influence Factor VIII binding .
	manualset3
212326	4	419497	7	NULL	NULL	0	NULL	Factor VIII	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In a competition assay , fluid-phase flvWF appeared to inhibit efficiently the binding of Factor VIII to immobilized vWF isolated from plasma , whereas vWFdelpro did not influence Factor VIII binding .
	manualset3
212327	5	419497	7	NULL	NULL	0	NULL	immobilized vWF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In a competition assay , fluid-phase flvWF appeared to inhibit efficiently the binding of Factor VIII to immobilized vWF isolated from plasma , whereas vWFdelpro did not influence Factor VIII binding .
	manualset3
212328	6	419497	7	NULL	NULL	0	NULL	plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In a competition assay , fluid-phase flvWF appeared to inhibit efficiently the binding of Factor VIII to immobilized vWF isolated from plasma , whereas vWFdelpro did not influence Factor VIII binding .
	manualset3
212329	7	419497	7	NULL	NULL	0	NULL	vWFdelpro	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In a competition assay , fluid-phase flvWF appeared to inhibit efficiently the binding of Factor VIII to immobilized vWF isolated from plasma , whereas vWFdelpro did not influence Factor VIII binding .
	manualset3
212330	8	419497	7	NULL	NULL	0	NULL	Factor VIII binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In a competition assay , fluid-phase flvWF appeared to inhibit efficiently the binding of Factor VIII to immobilized vWF isolated from plasma , whereas vWFdelpro did not influence Factor VIII binding .
	manualset3
212331	1	419498	7	NULL	NULL	0	NULL	effort	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effort exerted on the driving tasks was assessed though self-report ( RSME ) , psychophysiological measures ( pupil dilation ) and visual gaze data .
	manualset3
212332	2	419498	7	NULL	NULL	0	NULL	driving tasks	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effort exerted on the driving tasks was assessed though self-report ( RSME ) , psychophysiological measures ( pupil dilation ) and visual gaze data .
	manualset3
212333	3	419498	7	NULL	NULL	0	NULL	self-report ( RSME ) 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The effort exerted on the driving tasks was assessed though self-report ( RSME ) , psychophysiological measures ( pupil dilation ) and visual gaze data .
	manualset3
212334	4	419498	7	NULL	NULL	0	NULL	psychophysiological measures 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effort exerted on the driving tasks was assessed though self-report ( RSME ) , psychophysiological measures ( pupil dilation ) and visual gaze data .
	manualset3
212335	5	419498	7	NULL	NULL	0	NULL	pupil dilation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effort exerted on the driving tasks was assessed though self-report ( RSME ) , psychophysiological measures ( pupil dilation ) and visual gaze data .
	manualset3
212336	6	419498	7	NULL	NULL	0	NULL	visual gaze data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The effort exerted on the driving tasks was assessed though self-report ( RSME ) , psychophysiological measures ( pupil dilation ) and visual gaze data .
	manualset3
212337	1	419499	7	NULL	NULL	0	NULL	compact optical head 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	A compact optical head based on our new objective lens capable of TB storage is described .
	manualset3
212338	2	419499	7	NULL	NULL	0	NULL	new objective lens	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	A compact optical head based on our new objective lens capable of TB storage is described .
	manualset3
212339	3	419499	7	NULL	NULL	0	NULL	TB storage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A compact optical head based on our new objective lens capable of TB storage is described .
	manualset3
212340	1	419500	7	NULL	NULL	0	NULL	Effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Effect of histamine on the signal transduction of the AtoS-AtoC two component system and involvement in poly - ( R ) -3 - hydroxybutyrate biosynthesis in Escherichia coli .
	manualset3
212341	2	419500	7	NULL	NULL	0	NULL	histamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Effect of histamine on the signal transduction of the AtoS-AtoC two component system and involvement in poly - ( R ) -3 - hydroxybutyrate biosynthesis in Escherichia coli .
	manualset3
212342	3	419500	7	NULL	NULL	0	NULL	 signal transduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Effect of histamine on the signal transduction of the AtoS-AtoC two component system and involvement in poly - ( R ) -3 - hydroxybutyrate biosynthesis in Escherichia coli .
	manualset3
212343	4	419500	7	NULL	NULL	0	NULL	 AtoS-AtoC two component system	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Effect of histamine on the signal transduction of the AtoS-AtoC two component system and involvement in poly - ( R ) -3 - hydroxybutyrate biosynthesis in Escherichia coli .
	manualset3
212344	5	419500	7	NULL	NULL	0	NULL	involvement	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Effect of histamine on the signal transduction of the AtoS-AtoC two component system and involvement in poly - ( R ) -3 - hydroxybutyrate biosynthesis in Escherichia coli .
	manualset3
212345	6	419500	7	NULL	NULL	0	NULL	poly - ( R ) -3 - hydroxybutyrate biosynthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Effect of histamine on the signal transduction of the AtoS-AtoC two component system and involvement in poly - ( R ) -3 - hydroxybutyrate biosynthesis in Escherichia coli .
	manualset3
212346	7	419500	7	NULL	NULL	0	NULL	Escherichia coli 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Effect of histamine on the signal transduction of the AtoS-AtoC two component system and involvement in poly - ( R ) -3 - hydroxybutyrate biosynthesis in Escherichia coli .
	manualset3
212347	1	419501	7	NULL	NULL	0	NULL	Dioxygen	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Dioxygen binds tightly to reduced flavohemoglobin , with association and dissociation rate constants equal to 38 microM ( -1 ) s ( -1 ) and 0.44 s ( -1 ) , respectively , and the oxygenated flavohemoglobin dioxygenates NO to form nitrate .
	manualset3
212348	2	419501	7	NULL	NULL	0	NULL	flavohemoglobin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Dioxygen binds tightly to reduced flavohemoglobin , with association and dissociation rate constants equal to 38 microM ( -1 ) s ( -1 ) and 0.44 s ( -1 ) , respectively , and the oxygenated flavohemoglobin dioxygenates NO to form nitrate .
	manualset3
212349	3	419501	7	NULL	NULL	NULL	NULL	association rate constants	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dioxygen binds tightly to reduced flavohemoglobin , with association and dissociation rate constants equal to 38 microM ( -1 ) s ( -1 ) and 0.44 s ( -1 ) , respectively , and the oxygenated flavohemoglobin dioxygenates NO to form nitrate .
	manualset3
212350	4	419501	7	NULL	NULL	0	NULL	dissociation rate constants	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dioxygen binds tightly to reduced flavohemoglobin , with association and dissociation rate constants equal to 38 microM ( -1 ) s ( -1 ) and 0.44 s ( -1 ) , respectively , and the oxygenated flavohemoglobin dioxygenates NO to form nitrate .
	manualset3
212351	5	419501	7	NULL	NULL	NULL	NULL	38 microM ( -1 ) s ( -1 )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dioxygen binds tightly to reduced flavohemoglobin , with association and dissociation rate constants equal to 38 microM ( -1 ) s ( -1 ) and 0.44 s ( -1 ) , respectively , and the oxygenated flavohemoglobin dioxygenates NO to form nitrate .
	manualset3
212352	6	419501	7	NULL	NULL	0	NULL	0.44 s ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Dioxygen binds tightly to reduced flavohemoglobin , with association and dissociation rate constants equal to 38 microM ( -1 ) s ( -1 ) and 0.44 s ( -1 ) , respectively , and the oxygenated flavohemoglobin dioxygenates NO to form nitrate .
	manualset3
212353	7	419501	7	NULL	NULL	0	NULL	oxygenated flavohemoglobin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Dioxygen binds tightly to reduced flavohemoglobin , with association and dissociation rate constants equal to 38 microM ( -1 ) s ( -1 ) and 0.44 s ( -1 ) , respectively , and the oxygenated flavohemoglobin dioxygenates NO to form nitrate .
	manualset3
212354	8	419501	7	NULL	NULL	0	NULL	NO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Dioxygen binds tightly to reduced flavohemoglobin , with association and dissociation rate constants equal to 38 microM ( -1 ) s ( -1 ) and 0.44 s ( -1 ) , respectively , and the oxygenated flavohemoglobin dioxygenates NO to form nitrate .
	manualset3
212355	9	419501	7	NULL	NULL	0	NULL	nitrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Dioxygen binds tightly to reduced flavohemoglobin , with association and dissociation rate constants equal to 38 microM ( -1 ) s ( -1 ) and 0.44 s ( -1 ) , respectively , and the oxygenated flavohemoglobin dioxygenates NO to form nitrate .
	manualset3
212356	1	419502	7	NULL	NULL	0	NULL	Orexin B immunoreactive fibers 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Orexin B immunoreactive fibers and terminals innervate the sensory and motor neurons of jaw-elevator muscles in the rat .
	manualset3
212357	2	419502	7	NULL	NULL	0	NULL	 terminals	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Orexin B immunoreactive fibers and terminals innervate the sensory and motor neurons of jaw-elevator muscles in the rat .
	manualset3
212358	3	419502	7	NULL	NULL	0	NULL	sensory neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Orexin B immunoreactive fibers and terminals innervate the sensory and motor neurons of jaw-elevator muscles in the rat .
	manualset3
212359	4	419502	7	NULL	NULL	0	NULL	motor neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Orexin B immunoreactive fibers and terminals innervate the sensory and motor neurons of jaw-elevator muscles in the rat .
	manualset3
212360	5	419502	7	NULL	NULL	0	NULL	jaw-elevator muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Orexin B immunoreactive fibers and terminals innervate the sensory and motor neurons of jaw-elevator muscles in the rat .
	manualset3
212361	6	419502	7	NULL	NULL	0	NULL	rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Orexin B immunoreactive fibers and terminals innervate the sensory and motor neurons of jaw-elevator muscles in the rat .
	manualset3
212362	1	419503	7	NULL	NULL	0	NULL	 50 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although more than 50 % of the respondents had taken courses in education , many felt inadequately prepared for their role .
	manualset3
212363	2	419503	7	NULL	NULL	0	NULL	 respondents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although more than 50 % of the respondents had taken courses in education , many felt inadequately prepared for their role .
	manualset3
212364	3	419503	7	NULL	NULL	0	NULL	courses	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Although more than 50 % of the respondents had taken courses in education , many felt inadequately prepared for their role .
	manualset3
212365	4	419503	7	NULL	NULL	0	NULL	education	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Although more than 50 % of the respondents had taken courses in education , many felt inadequately prepared for their role .
	manualset3
212366	5	419503	7	NULL	NULL	NULL	NULL	role	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although more than 50 % of the respondents had taken courses in education , many felt inadequately prepared for their role .
	manualset3
212367	1	419504	7	NULL	NULL	0	NULL	capacity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrated the capacity of the loop to disrupt the interaction between Mg ( 2 + ) - ATP complex and the N-domain and propose a role for this loop in the allosteric regulation of the nucleotide binding process .
	manualset3
212368	2	419504	7	NULL	NULL	NULL	NULL	 loop	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We demonstrated the capacity of the loop to disrupt the interaction between Mg ( 2 + ) - ATP complex and the N-domain and propose a role for this loop in the allosteric regulation of the nucleotide binding process .
	manualset3
212369	3	419504	7	NULL	NULL	0	NULL	 interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrated the capacity of the loop to disrupt the interaction between Mg ( 2 + ) - ATP complex and the N-domain and propose a role for this loop in the allosteric regulation of the nucleotide binding process .
	manualset3
212370	4	419504	7	NULL	NULL	0	NULL	Mg ( 2 + ) - ATP complex	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrated the capacity of the loop to disrupt the interaction between Mg ( 2 + ) - ATP complex and the N-domain and propose a role for this loop in the allosteric regulation of the nucleotide binding process .
	manualset3
212371	5	419504	7	NULL	NULL	0	NULL	N-domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrated the capacity of the loop to disrupt the interaction between Mg ( 2 + ) - ATP complex and the N-domain and propose a role for this loop in the allosteric regulation of the nucleotide binding process .
	manualset3
212372	6	419504	7	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrated the capacity of the loop to disrupt the interaction between Mg ( 2 + ) - ATP complex and the N-domain and propose a role for this loop in the allosteric regulation of the nucleotide binding process .
	manualset3
212373	7	419504	7	NULL	NULL	0	NULL	loop	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrated the capacity of the loop to disrupt the interaction between Mg ( 2 + ) - ATP complex and the N-domain and propose a role for this loop in the allosteric regulation of the nucleotide binding process .
	manualset3
212374	8	419504	7	NULL	NULL	0	NULL	allosteric regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrated the capacity of the loop to disrupt the interaction between Mg ( 2 + ) - ATP complex and the N-domain and propose a role for this loop in the allosteric regulation of the nucleotide binding process .
	manualset3
212375	9	419504	7	NULL	NULL	0	NULL	nucleotide binding process	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrated the capacity of the loop to disrupt the interaction between Mg ( 2 + ) - ATP complex and the N-domain and propose a role for this loop in the allosteric regulation of the nucleotide binding process .
	manualset3
212376	1	419505	7	NULL	NULL	0	NULL	 war	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Does war prevent the spread of HIV ?
	manualset3
212377	2	419505	7	NULL	NULL	0	NULL	spread of HIV	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Does war prevent the spread of HIV ?
	manualset3
212378	1	419506	7	NULL	NULL	0	NULL	Fly mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Fly mortality increased rapidly after 2 h of anoxia and & gt ; 16 h exposure was uniformly lethal .
	manualset3
212379	2	419506	7	NULL	NULL	0	NULL	 2 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Fly mortality increased rapidly after 2 h of anoxia and & gt ; 16 h exposure was uniformly lethal .
	manualset3
212380	3	419506	7	NULL	NULL	0	NULL	anoxia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Fly mortality increased rapidly after 2 h of anoxia and & gt ; 16 h exposure was uniformly lethal .
	manualset3
212381	4	419506	7	NULL	NULL	0	NULL	& gt	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Fly mortality increased rapidly after 2 h of anoxia and & gt ; 16 h exposure was uniformly lethal .
	manualset3
212382	5	419506	7	NULL	NULL	0	NULL	 16 h exposure	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Fly mortality increased rapidly after 2 h of anoxia and & gt ; 16 h exposure was uniformly lethal .
	manualset3
212383	6	419506	7	NULL	NULL	NULL	NULL	lethal	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fly mortality increased rapidly after 2 h of anoxia and & gt ; 16 h exposure was uniformly lethal .
	manualset3
212384	1	419507	7	NULL	NULL	0	NULL	Isolation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation and preliminary characterization of that part of the plasma membrane which is apposed to the substratum .
	manualset3
212385	2	419507	7	NULL	NULL	0	NULL	 preliminary characterization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation and preliminary characterization of that part of the plasma membrane which is apposed to the substratum .
	manualset3
212386	3	419507	7	NULL	NULL	0	NULL	part of the plasma membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation and preliminary characterization of that part of the plasma membrane which is apposed to the substratum .
	manualset3
212387	4	419507	7	NULL	NULL	0	NULL	substratum	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation and preliminary characterization of that part of the plasma membrane which is apposed to the substratum .
	manualset3
212388	1	419508	7	NULL	NULL	0	NULL	Percutaneous cystolithotomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Percutaneous cystolithotomy for vesical calculi : a better approach .
	manualset3
212389	2	419508	7	NULL	NULL	0	NULL	vesical calculi	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Percutaneous cystolithotomy for vesical calculi : a better approach .
	manualset3
212390	3	419508	7	NULL	NULL	0	NULL	better approach	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Percutaneous cystolithotomy for vesical calculi : a better approach .
	manualset3
212391	1	419509	7	NULL	NULL	0	NULL	Purification 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification of the active lipid was achieved by chloroform-methanol extraction of the whole organisms yielding a chloroform-soluble fraction attracting mononuclear phagocytes at concentrations around 10 microgram/ml .
	manualset3
212434	2	419509	7	NULL	NULL	0	NULL	active lipid	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification of the active lipid was achieved by chloroform-methanol extraction of the whole organisms yielding a chloroform-soluble fraction attracting mononuclear phagocytes at concentrations around 10 microgram/ml .
	manualset3
212435	3	419509	7	NULL	NULL	0	NULL	 chloroform-methanol extraction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification of the active lipid was achieved by chloroform-methanol extraction of the whole organisms yielding a chloroform-soluble fraction attracting mononuclear phagocytes at concentrations around 10 microgram/ml .
	manualset3
212436	4	419509	7	NULL	NULL	0	NULL	whole organisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification of the active lipid was achieved by chloroform-methanol extraction of the whole organisms yielding a chloroform-soluble fraction attracting mononuclear phagocytes at concentrations around 10 microgram/ml .
	manualset3
212437	5	419509	7	NULL	NULL	0	NULL	chloroform-soluble fraction	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification of the active lipid was achieved by chloroform-methanol extraction of the whole organisms yielding a chloroform-soluble fraction attracting mononuclear phagocytes at concentrations around 10 microgram/ml .
	manualset3
212438	6	419509	7	NULL	NULL	0	NULL	mononuclear phagocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification of the active lipid was achieved by chloroform-methanol extraction of the whole organisms yielding a chloroform-soluble fraction attracting mononuclear phagocytes at concentrations around 10 microgram/ml .
	manualset3
212439	7	419509	7	NULL	NULL	0	NULL	concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification of the active lipid was achieved by chloroform-methanol extraction of the whole organisms yielding a chloroform-soluble fraction attracting mononuclear phagocytes at concentrations around 10 microgram/ml .
	manualset3
212440	8	419509	7	NULL	NULL	0	NULL	10 microgram/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification of the active lipid was achieved by chloroform-methanol extraction of the whole organisms yielding a chloroform-soluble fraction attracting mononuclear phagocytes at concentrations around 10 microgram/ml .
	manualset3
212441	1	419510	7	NULL	NULL	0	NULL	Production 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of tense morphology by Afrikaans-speaking children with and without specific language impairment .
	manualset3
212442	2	419510	7	NULL	NULL	0	NULL	tense morphology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of tense morphology by Afrikaans-speaking children with and without specific language impairment .
	manualset3
212443	3	419510	7	NULL	NULL	0	NULL	Afrikaans-speaking children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of tense morphology by Afrikaans-speaking children with and without specific language impairment .
	manualset3
212444	4	419510	7	NULL	NULL	0	NULL	language impairment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Production of tense morphology by Afrikaans-speaking children with and without specific language impairment .
	manualset3
212445	1	419511	7	NULL	NULL	0	NULL	Mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of formation of linolenic acid radicals and their role in initiation of peroxidation were studied .
	manualset3
212446	2	419511	7	NULL	NULL	0	NULL	formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of formation of linolenic acid radicals and their role in initiation of peroxidation were studied .
	manualset3
212447	3	419511	7	NULL	NULL	0	NULL	linolenic acid radicals	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of formation of linolenic acid radicals and their role in initiation of peroxidation were studied .
	manualset3
212448	4	419511	7	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of formation of linolenic acid radicals and their role in initiation of peroxidation were studied .
	manualset3
212449	5	419511	7	NULL	NULL	0	NULL	initiation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of formation of linolenic acid radicals and their role in initiation of peroxidation were studied .
	manualset3
212450	6	419511	7	NULL	NULL	0	NULL	peroxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mechanism of formation of linolenic acid radicals and their role in initiation of peroxidation were studied .
	manualset3
212451	1	419512	7	NULL	NULL	0	NULL	Active treatment modalities	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Active treatment modalities are clearly indicated in varices with complications such as trophic skin changes , varicophlebitis or when varices cause pain .
	manualset3
212452	2	419512	7	NULL	NULL	0	NULL	complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Active treatment modalities are clearly indicated in varices with complications such as trophic skin changes , varicophlebitis or when varices cause pain .
	manualset3
212453	3	419512	7	NULL	NULL	0	NULL	trophic skin changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Active treatment modalities are clearly indicated in varices with complications such as trophic skin changes , varicophlebitis or when varices cause pain .
	manualset3
212454	4	419512	7	NULL	NULL	0	NULL	varicophlebitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Active treatment modalities are clearly indicated in varices with complications such as trophic skin changes , varicophlebitis or when varices cause pain .
	manualset3
212455	5	419512	7	NULL	NULL	0	NULL	varices	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Active treatment modalities are clearly indicated in varices with complications such as trophic skin changes , varicophlebitis or when varices cause pain .
	manualset3
212456	6	419512	7	NULL	NULL	0	NULL	pain 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Active treatment modalities are clearly indicated in varices with complications such as trophic skin changes , varicophlebitis or when varices cause pain .
	manualset3
212457	7	419512	7	NULL	NULL	0	NULL	varices	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Active treatment modalities are clearly indicated in varices with complications such as trophic skin changes , varicophlebitis or when varices cause pain .
	manualset3
212597	1	419514	7	NULL	NULL	0	NULL	N desulphated N acetylated CY 142	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	N desulphated N acetylated CY 142 and CY 143 had no effect .
	manualset3
212598	2	419514	7	NULL	NULL	0	NULL	N desulphated N acetylated CY 143	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	N desulphated N acetylated CY 142 and CY 143 had no effect .
	manualset3
212599	3	419514	7	NULL	NULL	0	NULL	no effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	N desulphated N acetylated CY 142 and CY 143 had no effect .
	manualset3
212600	1	419515	7	NULL	NULL	0	NULL	Phosphonoacetohydroxamic acid ( PhAH )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphonoacetohydroxamic acid ( PhAH ) was found to be a strong competitive inhibitor ( K ( i ) = 5.1 + / - 1.6 microM ) whereas phosphonoacetic acid ( K ( i ) = 380 + / - 45 microM ) and acetohydroxamic acid ( K ( i ) ) 75 mM ) modestly inhibited lambdaPP .
	manualset3
212601	2	419515	7	NULL	NULL	0	NULL	strong competitive inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphonoacetohydroxamic acid ( PhAH ) was found to be a strong competitive inhibitor ( K ( i ) = 5.1 + / - 1.6 microM ) whereas phosphonoacetic acid ( K ( i ) = 380 + / - 45 microM ) and acetohydroxamic acid ( K ( i ) ) 75 mM ) modestly inhibited lambdaPP .
	manualset3
212602	3	419515	7	NULL	NULL	0	NULL	K ( i ) = 5.1 + / - 1.6 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphonoacetohydroxamic acid ( PhAH ) was found to be a strong competitive inhibitor ( K ( i ) = 5.1 + / - 1.6 microM ) whereas phosphonoacetic acid ( K ( i ) = 380 + / - 45 microM ) and acetohydroxamic acid ( K ( i ) ) 75 mM ) modestly inhibited lambdaPP .
	manualset3
212603	4	419515	7	NULL	NULL	0	NULL	phosphonoacetic acid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphonoacetohydroxamic acid ( PhAH ) was found to be a strong competitive inhibitor ( K ( i ) = 5.1 + / - 1.6 microM ) whereas phosphonoacetic acid ( K ( i ) = 380 + / - 45 microM ) and acetohydroxamic acid ( K ( i ) ) 75 mM ) modestly inhibited lambdaPP .
	manualset3
212604	5	419515	7	NULL	NULL	0	NULL	K ( i ) = 380 + / - 45 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphonoacetohydroxamic acid ( PhAH ) was found to be a strong competitive inhibitor ( K ( i ) = 5.1 + / - 1.6 microM ) whereas phosphonoacetic acid ( K ( i ) = 380 + / - 45 microM ) and acetohydroxamic acid ( K ( i ) ) 75 mM ) modestly inhibited lambdaPP .
	manualset3
212605	6	419515	7	NULL	NULL	0	NULL	acetohydroxamic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphonoacetohydroxamic acid ( PhAH ) was found to be a strong competitive inhibitor ( K ( i ) = 5.1 + / - 1.6 microM ) whereas phosphonoacetic acid ( K ( i ) = 380 + / - 45 microM ) and acetohydroxamic acid ( K ( i ) ) 75 mM ) modestly inhibited lambdaPP .
	manualset3
212606	7	419515	7	NULL	NULL	0	NULL	K ( i ) ) 75 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphonoacetohydroxamic acid ( PhAH ) was found to be a strong competitive inhibitor ( K ( i ) = 5.1 + / - 1.6 microM ) whereas phosphonoacetic acid ( K ( i ) = 380 + / - 45 microM ) and acetohydroxamic acid ( K ( i ) ) 75 mM ) modestly inhibited lambdaPP .
	manualset3
212607	8	419515	7	NULL	NULL	NULL	NULL	lambdaPP	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Phosphonoacetohydroxamic acid ( PhAH ) was found to be a strong competitive inhibitor ( K ( i ) = 5.1 + / - 1.6 microM ) whereas phosphonoacetic acid ( K ( i ) = 380 + / - 45 microM ) and acetohydroxamic acid ( K ( i ) ) 75 mM ) modestly inhibited lambdaPP .
	manualset3
212608	1	419516	7	NULL	NULL	0	NULL	 complex	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the complex , each thio-cyanate anion functions as a bridging ligand , linking adjacent Cd ( II ) ions with a separation of 6.4919 ( 6 ) , resulting in the formation of a two-dimensional sheet structure in the bc plane .
	manualset3
212609	2	419516	7	NULL	NULL	0	NULL	 thio-cyanate anion	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In the complex , each thio-cyanate anion functions as a bridging ligand , linking adjacent Cd ( II ) ions with a separation of 6.4919 ( 6 ) , resulting in the formation of a two-dimensional sheet structure in the bc plane .
	manualset3
212610	3	419516	7	NULL	NULL	0	NULL	bridging ligand	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the complex , each thio-cyanate anion functions as a bridging ligand , linking adjacent Cd ( II ) ions with a separation of 6.4919 ( 6 ) , resulting in the formation of a two-dimensional sheet structure in the bc plane .
	manualset3
212611	4	419516	7	NULL	NULL	0	NULL	Cd ( II ) ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In the complex , each thio-cyanate anion functions as a bridging ligand , linking adjacent Cd ( II ) ions with a separation of 6.4919 ( 6 ) , resulting in the formation of a two-dimensional sheet structure in the bc plane .
	manualset3
212612	5	419516	7	NULL	NULL	0	NULL	separation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the complex , each thio-cyanate anion functions as a bridging ligand , linking adjacent Cd ( II ) ions with a separation of 6.4919 ( 6 ) , resulting in the formation of a two-dimensional sheet structure in the bc plane .
	manualset3
212613	6	419516	7	NULL	NULL	0	NULL	6.4919 ( 6 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the complex , each thio-cyanate anion functions as a bridging ligand , linking adjacent Cd ( II ) ions with a separation of 6.4919 ( 6 ) , resulting in the formation of a two-dimensional sheet structure in the bc plane .
	manualset3
212614	7	419516	7	NULL	NULL	0	NULL	formation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the complex , each thio-cyanate anion functions as a bridging ligand , linking adjacent Cd ( II ) ions with a separation of 6.4919 ( 6 ) , resulting in the formation of a two-dimensional sheet structure in the bc plane .
	manualset3
212615	8	419516	7	NULL	NULL	0	NULL	two-dimensional sheet structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the complex , each thio-cyanate anion functions as a bridging ligand , linking adjacent Cd ( II ) ions with a separation of 6.4919 ( 6 ) , resulting in the formation of a two-dimensional sheet structure in the bc plane .
	manualset3
212616	9	419516	7	NULL	NULL	0	NULL	bc plane	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In the complex , each thio-cyanate anion functions as a bridging ligand , linking adjacent Cd ( II ) ions with a separation of 6.4919 ( 6 ) , resulting in the formation of a two-dimensional sheet structure in the bc plane .
	manualset3
212617	1	419517	7	NULL	NULL	0	NULL	Baetis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Baetis and Pentaneura were scarce , and Asellus absent , in remnant Gammarus treatments , as a consequence of interference and/or predation by the amphipods .
	manualset3
212618	2	419517	7	NULL	NULL	0	NULL	Pentaneura	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Baetis and Pentaneura were scarce , and Asellus absent , in remnant Gammarus treatments , as a consequence of interference and/or predation by the amphipods .
	manualset3
212619	3	419517	7	NULL	NULL	0	NULL	Asellus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Baetis and Pentaneura were scarce , and Asellus absent , in remnant Gammarus treatments , as a consequence of interference and/or predation by the amphipods .
	manualset3
212620	4	419517	7	NULL	NULL	0	NULL	Gammarus treatments	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Baetis and Pentaneura were scarce , and Asellus absent , in remnant Gammarus treatments , as a consequence of interference and/or predation by the amphipods .
	manualset3
212621	5	419517	7	NULL	NULL	0	NULL	predation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Baetis and Pentaneura were scarce , and Asellus absent , in remnant Gammarus treatments , as a consequence of interference and/or predation by the amphipods .
	manualset3
212622	6	419517	7	NULL	NULL	0	NULL	amphipods	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Baetis and Pentaneura were scarce , and Asellus absent , in remnant Gammarus treatments , as a consequence of interference and/or predation by the amphipods .
	manualset3
214134	7	419517	7	NULL	NULL	0	NULL	interference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Baetis and Pentaneura were scarce , and Asellus absent , in remnant Gammarus treatments , as a consequence of interference and/or predation by the amphipods .
	manualset3
212628	1	419518	7	NULL	NULL	0	NULL	Angioimmunoblastic T-Cell Lymphoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Is the Angioimmunoblastic T-Cell Lymphoma Beneficial to Avoid CD4 ( + ) Lymphopenia and Other AIDS Manifestations in Patients Infected With Human Immunodeficiency Virus ?
	manualset3
212630	2	419518	7	NULL	NULL	0	NULL	CD4 ( + ) Lymphopenia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Is the Angioimmunoblastic T-Cell Lymphoma Beneficial to Avoid CD4 ( + ) Lymphopenia and Other AIDS Manifestations in Patients Infected With Human Immunodeficiency Virus ?
	manualset3
212632	3	419518	7	NULL	NULL	0	NULL	AIDS Manifestations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Is the Angioimmunoblastic T-Cell Lymphoma Beneficial to Avoid CD4 ( + ) Lymphopenia and Other AIDS Manifestations in Patients Infected With Human Immunodeficiency Virus ?
	manualset3
212633	4	419518	7	NULL	NULL	0	NULL	Patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Is the Angioimmunoblastic T-Cell Lymphoma Beneficial to Avoid CD4 ( + ) Lymphopenia and Other AIDS Manifestations in Patients Infected With Human Immunodeficiency Virus ?
	manualset3
212636	5	419518	7	NULL	NULL	0	NULL	Human Immunodeficiency Virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Is the Angioimmunoblastic T-Cell Lymphoma Beneficial to Avoid CD4 ( + ) Lymphopenia and Other AIDS Manifestations in Patients Infected With Human Immunodeficiency Virus ?
	manualset3
212639	1	419519	7	NULL	NULL	0	NULL	Objectives	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Objectives : Our purpose was to analyze longitudinal relationships between older spouses ' cognitive function and the cognitive function of their partners 5 years later , as well as to assess moderating roles of gender and marital quality .
	manualset3
212640	2	419519	7	NULL	NULL	0	NULL	purpose	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Objectives : Our purpose was to analyze longitudinal relationships between older spouses ' cognitive function and the cognitive function of their partners 5 years later , as well as to assess moderating roles of gender and marital quality .
	manualset3
212643	3	419519	7	NULL	NULL	0	NULL	longitudinal relationships 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Objectives : Our purpose was to analyze longitudinal relationships between older spouses ' cognitive function and the cognitive function of their partners 5 years later , as well as to assess moderating roles of gender and marital quality .
	manualset3
212644	4	419519	7	NULL	NULL	0	NULL	older spouses ' cognitive function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Objectives : Our purpose was to analyze longitudinal relationships between older spouses ' cognitive function and the cognitive function of their partners 5 years later , as well as to assess moderating roles of gender and marital quality .
	manualset3
212645	5	419519	7	NULL	NULL	0	NULL	cognitive function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Objectives : Our purpose was to analyze longitudinal relationships between older spouses ' cognitive function and the cognitive function of their partners 5 years later , as well as to assess moderating roles of gender and marital quality .
	manualset3
212648	6	419519	7	NULL	NULL	0	NULL	partners	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Objectives : Our purpose was to analyze longitudinal relationships between older spouses ' cognitive function and the cognitive function of their partners 5 years later , as well as to assess moderating roles of gender and marital quality .
	manualset3
212651	7	419519	7	NULL	NULL	0	NULL	 5 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Objectives : Our purpose was to analyze longitudinal relationships between older spouses ' cognitive function and the cognitive function of their partners 5 years later , as well as to assess moderating roles of gender and marital quality .
	manualset3
212653	8	419519	7	NULL	NULL	0	NULL	moderating roles	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Objectives : Our purpose was to analyze longitudinal relationships between older spouses ' cognitive function and the cognitive function of their partners 5 years later , as well as to assess moderating roles of gender and marital quality .
	manualset3
212654	9	419519	7	NULL	NULL	0	NULL	gender	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Objectives : Our purpose was to analyze longitudinal relationships between older spouses ' cognitive function and the cognitive function of their partners 5 years later , as well as to assess moderating roles of gender and marital quality .
	manualset3
212655	10	419519	7	NULL	NULL	0	NULL	marital quality	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Objectives : Our purpose was to analyze longitudinal relationships between older spouses ' cognitive function and the cognitive function of their partners 5 years later , as well as to assess moderating roles of gender and marital quality .
	manualset3
212656	1	419520	7	NULL	NULL	0	NULL	Madness 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Madness '' and `` eccentricities '' perpetuated by Old School medical craftsmen are prevalent today in the strange practices of the new charlatanism , such as trunk cell technologies .
	manualset3
212657	2	419520	7	NULL	NULL	0	NULL	eccentricities	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Madness '' and `` eccentricities '' perpetuated by Old School medical craftsmen are prevalent today in the strange practices of the new charlatanism , such as trunk cell technologies .
	manualset3
212658	3	419520	7	NULL	NULL	0	NULL	Old School medical craftsmen	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Madness '' and `` eccentricities '' perpetuated by Old School medical craftsmen are prevalent today in the strange practices of the new charlatanism , such as trunk cell technologies .
	manualset3
212659	4	419520	7	NULL	NULL	0	NULL	today	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Madness '' and `` eccentricities '' perpetuated by Old School medical craftsmen are prevalent today in the strange practices of the new charlatanism , such as trunk cell technologies .
	manualset3
212661	5	419520	7	NULL	NULL	0	NULL	 strange practices	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Madness '' and `` eccentricities '' perpetuated by Old School medical craftsmen are prevalent today in the strange practices of the new charlatanism , such as trunk cell technologies .
	manualset3
212664	6	419520	7	NULL	NULL	0	NULL	new charlatanism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Madness '' and `` eccentricities '' perpetuated by Old School medical craftsmen are prevalent today in the strange practices of the new charlatanism , such as trunk cell technologies .
	manualset3
212665	7	419520	7	NULL	NULL	0	NULL	trunk cell technologies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Madness '' and `` eccentricities '' perpetuated by Old School medical craftsmen are prevalent today in the strange practices of the new charlatanism , such as trunk cell technologies .
	manualset3
212666	1	419521	7	NULL	NULL	0	NULL	good outcome 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The good outcome , as verified by arteriography , and the experience of other groups , makes it clear that there is a specific place for this therapy in such patients .
	manualset3
212667	2	419521	7	NULL	NULL	0	NULL	arteriography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The good outcome , as verified by arteriography , and the experience of other groups , makes it clear that there is a specific place for this therapy in such patients .
	manualset3
212668	3	419521	7	NULL	NULL	0	NULL	experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The good outcome , as verified by arteriography , and the experience of other groups , makes it clear that there is a specific place for this therapy in such patients .
	manualset3
212669	4	419521	7	NULL	NULL	0	NULL	groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The good outcome , as verified by arteriography , and the experience of other groups , makes it clear that there is a specific place for this therapy in such patients .
	manualset3
212670	5	419521	7	NULL	NULL	0	NULL	 place	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The good outcome , as verified by arteriography , and the experience of other groups , makes it clear that there is a specific place for this therapy in such patients .
	manualset3
212671	6	419521	7	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The good outcome , as verified by arteriography , and the experience of other groups , makes it clear that there is a specific place for this therapy in such patients .
	manualset3
212672	7	419521	7	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The good outcome , as verified by arteriography , and the experience of other groups , makes it clear that there is a specific place for this therapy in such patients .
	manualset3
212673	1	419522	7	NULL	NULL	0	NULL	Adult medium mode	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Adult medium mode gave significantly higher results than pediatric large mode for total body fat mass ( 11.1 % ) , fat % ( 10.5 % ) , bone mineral content ( 8.1 % ) , and bone area ( 1.3 % ) ( p & lt ; 0.02 ) .
	manualset3
212674	2	419522	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Adult medium mode gave significantly higher results than pediatric large mode for total body fat mass ( 11.1 % ) , fat % ( 10.5 % ) , bone mineral content ( 8.1 % ) , and bone area ( 1.3 % ) ( p & lt ; 0.02 ) .
	manualset3
212675	3	419522	7	NULL	NULL	NULL	NULL	pediatric large mode	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Adult medium mode gave significantly higher results than pediatric large mode for total body fat mass ( 11.1 % ) , fat % ( 10.5 % ) , bone mineral content ( 8.1 % ) , and bone area ( 1.3 % ) ( p & lt ; 0.02 ) .
	manualset3
212676	4	419522	7	NULL	NULL	0	NULL	total body fat mass 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Adult medium mode gave significantly higher results than pediatric large mode for total body fat mass ( 11.1 % ) , fat % ( 10.5 % ) , bone mineral content ( 8.1 % ) , and bone area ( 1.3 % ) ( p & lt ; 0.02 ) .
	manualset3
212677	5	419522	7	NULL	NULL	0	NULL	11.1 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Adult medium mode gave significantly higher results than pediatric large mode for total body fat mass ( 11.1 % ) , fat % ( 10.5 % ) , bone mineral content ( 8.1 % ) , and bone area ( 1.3 % ) ( p & lt ; 0.02 ) .
	manualset3
212678	6	419522	7	NULL	NULL	0	NULL	fat %	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Adult medium mode gave significantly higher results than pediatric large mode for total body fat mass ( 11.1 % ) , fat % ( 10.5 % ) , bone mineral content ( 8.1 % ) , and bone area ( 1.3 % ) ( p & lt ; 0.02 ) .
	manualset3
212680	7	419522	7	NULL	NULL	0	NULL	10.5 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Adult medium mode gave significantly higher results than pediatric large mode for total body fat mass ( 11.1 % ) , fat % ( 10.5 % ) , bone mineral content ( 8.1 % ) , and bone area ( 1.3 % ) ( p & lt ; 0.02 ) .
	manualset3
212681	8	419522	7	NULL	NULL	0	NULL	bone mineral content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Adult medium mode gave significantly higher results than pediatric large mode for total body fat mass ( 11.1 % ) , fat % ( 10.5 % ) , bone mineral content ( 8.1 % ) , and bone area ( 1.3 % ) ( p & lt ; 0.02 ) .
	manualset3
212682	9	419522	7	NULL	NULL	0	NULL	 8.1 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Adult medium mode gave significantly higher results than pediatric large mode for total body fat mass ( 11.1 % ) , fat % ( 10.5 % ) , bone mineral content ( 8.1 % ) , and bone area ( 1.3 % ) ( p & lt ; 0.02 ) .
	manualset3
212685	10	419522	7	NULL	NULL	0	NULL	bone area	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Adult medium mode gave significantly higher results than pediatric large mode for total body fat mass ( 11.1 % ) , fat % ( 10.5 % ) , bone mineral content ( 8.1 % ) , and bone area ( 1.3 % ) ( p & lt ; 0.02 ) .
	manualset3
212687	11	419522	7	NULL	NULL	0	NULL	1.3 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Adult medium mode gave significantly higher results than pediatric large mode for total body fat mass ( 11.1 % ) , fat % ( 10.5 % ) , bone mineral content ( 8.1 % ) , and bone area ( 1.3 % ) ( p & lt ; 0.02 ) .
	manualset3
212688	12	419522	7	NULL	NULL	0	NULL	p & lt ; 0.02	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Adult medium mode gave significantly higher results than pediatric large mode for total body fat mass ( 11.1 % ) , fat % ( 10.5 % ) , bone mineral content ( 8.1 % ) , and bone area ( 1.3 % ) ( p & lt ; 0.02 ) .
	manualset3
212690	1	419523	7	NULL	NULL	0	NULL	Tubular nuclear accumulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Tubular nuclear accumulation of Snail and epithelial phenotypic changes in human myeloma cast nephropathy .
	manualset3
212691	2	419523	7	NULL	NULL	0	NULL	 Snail	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Tubular nuclear accumulation of Snail and epithelial phenotypic changes in human myeloma cast nephropathy .
	manualset3
212692	3	419523	7	NULL	NULL	0	NULL	epithelial phenotypic changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Tubular nuclear accumulation of Snail and epithelial phenotypic changes in human myeloma cast nephropathy .
	manualset3
212693	4	419523	7	NULL	NULL	0	NULL	human myeloma cast nephropathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Tubular nuclear accumulation of Snail and epithelial phenotypic changes in human myeloma cast nephropathy .
	manualset3
212694	1	419524	7	NULL	NULL	0	NULL	recent study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A recent study reveals that casein kinase Iepsilon mediates an additional novel non-canonical Wnt pathway via the activation of the Rap1 GTPase during vertebrate gastrulation .
	manualset3
212695	2	419524	7	NULL	NULL	0	NULL	casein kinase Iepsilon	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A recent study reveals that casein kinase Iepsilon mediates an additional novel non-canonical Wnt pathway via the activation of the Rap1 GTPase during vertebrate gastrulation .
	manualset3
212696	3	419524	7	NULL	NULL	0	NULL	novel non-canonical Wnt pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A recent study reveals that casein kinase Iepsilon mediates an additional novel non-canonical Wnt pathway via the activation of the Rap1 GTPase during vertebrate gastrulation .
	manualset3
212697	4	419524	7	NULL	NULL	0	NULL	activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A recent study reveals that casein kinase Iepsilon mediates an additional novel non-canonical Wnt pathway via the activation of the Rap1 GTPase during vertebrate gastrulation .
	manualset3
212698	5	419524	7	NULL	NULL	0	NULL	Rap1 GTPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A recent study reveals that casein kinase Iepsilon mediates an additional novel non-canonical Wnt pathway via the activation of the Rap1 GTPase during vertebrate gastrulation .
	manualset3
212699	6	419524	7	NULL	NULL	0	NULL	vertebrate gastrulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A recent study reveals that casein kinase Iepsilon mediates an additional novel non-canonical Wnt pathway via the activation of the Rap1 GTPase during vertebrate gastrulation .
	manualset3
212700	1	419525	7	NULL	NULL	0	NULL	glycoconjugate purification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to optimize the glycoconjugate purification to complete functional and therapeutic studies , we have designed an improved method consisting of anion-exchange chromatography and reversed-phase HPLC , which can be easily scaled-up .
	manualset3
212714	2	419525	7	NULL	NULL	0	NULL	functional studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to optimize the glycoconjugate purification to complete functional and therapeutic studies , we have designed an improved method consisting of anion-exchange chromatography and reversed-phase HPLC , which can be easily scaled-up .
	manualset3
212716	3	419525	7	NULL	NULL	0	NULL	therapeutic studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to optimize the glycoconjugate purification to complete functional and therapeutic studies , we have designed an improved method consisting of anion-exchange chromatography and reversed-phase HPLC , which can be easily scaled-up .
	manualset3
212717	4	419525	7	NULL	NULL	0	NULL	improved method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to optimize the glycoconjugate purification to complete functional and therapeutic studies , we have designed an improved method consisting of anion-exchange chromatography and reversed-phase HPLC , which can be easily scaled-up .
	manualset3
212719	5	419525	7	NULL	NULL	0	NULL	anion-exchange chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to optimize the glycoconjugate purification to complete functional and therapeutic studies , we have designed an improved method consisting of anion-exchange chromatography and reversed-phase HPLC , which can be easily scaled-up .
	manualset3
212721	6	419525	7	NULL	NULL	0	NULL	reversed-phase HPLC	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to optimize the glycoconjugate purification to complete functional and therapeutic studies , we have designed an improved method consisting of anion-exchange chromatography and reversed-phase HPLC , which can be easily scaled-up .
	manualset3
212725	1	419526	7	NULL	NULL	0	NULL	 weak activity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It showed weak activity against Bauberia bassiana , an insect pathogenic fungus , and Staphylococcus aureus , a pathogenic bacterium .
	manualset3
212726	2	419526	7	NULL	NULL	0	NULL	Bauberia bassiana 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It showed weak activity against Bauberia bassiana , an insect pathogenic fungus , and Staphylococcus aureus , a pathogenic bacterium .
	manualset3
212728	3	419526	7	NULL	NULL	0	NULL	insect pathogenic fungus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It showed weak activity against Bauberia bassiana , an insect pathogenic fungus , and Staphylococcus aureus , a pathogenic bacterium .
	manualset3
212730	4	419526	7	NULL	NULL	0	NULL	Staphylococcus aureus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It showed weak activity against Bauberia bassiana , an insect pathogenic fungus , and Staphylococcus aureus , a pathogenic bacterium .
	manualset3
212732	5	419526	7	NULL	NULL	0	NULL	pathogenic bacterium	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It showed weak activity against Bauberia bassiana , an insect pathogenic fungus , and Staphylococcus aureus , a pathogenic bacterium .
	manualset3
212755	1	419527	7	NULL	NULL	0	NULL	neurologists 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although neurologists will not be the first responders to CBEs , they must know about the neurological effects in order to provide diagnosis and treatment to survivors .
	manualset3
212756	2	419527	7	NULL	NULL	0	NULL	first responders	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although neurologists will not be the first responders to CBEs , they must know about the neurological effects in order to provide diagnosis and treatment to survivors .
	manualset3
212764	3	419527	7	NULL	NULL	0	NULL	CBEs	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although neurologists will not be the first responders to CBEs , they must know about the neurological effects in order to provide diagnosis and treatment to survivors .
	manualset3
212766	4	419527	7	NULL	NULL	0	NULL	neurological effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although neurologists will not be the first responders to CBEs , they must know about the neurological effects in order to provide diagnosis and treatment to survivors .
	manualset3
212768	5	419527	7	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although neurologists will not be the first responders to CBEs , they must know about the neurological effects in order to provide diagnosis and treatment to survivors .
	manualset3
212770	6	419527	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Although neurologists will not be the first responders to CBEs , they must know about the neurological effects in order to provide diagnosis and treatment to survivors .
	manualset3
212772	7	419527	7	NULL	NULL	0	NULL	survivors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although neurologists will not be the first responders to CBEs , they must know about the neurological effects in order to provide diagnosis and treatment to survivors .
	manualset3
212774	1	419528	7	NULL	NULL	0	NULL	analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar analyses were repeated at day 7 following exposure to oxygen .
	manualset3
212775	2	419528	7	NULL	NULL	0	NULL	day 7	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar analyses were repeated at day 7 following exposure to oxygen .
	manualset3
212776	3	419528	7	NULL	NULL	0	NULL	exposure	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar analyses were repeated at day 7 following exposure to oxygen .
	manualset3
212777	4	419528	7	NULL	NULL	0	NULL	oxygen	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar analyses were repeated at day 7 following exposure to oxygen .
	manualset3
212785	1	419529	7	NULL	NULL	0	NULL	female patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A female patient was taken to the internal ward with a tentative diagnosis of recurrent syncope .
	manualset3
212786	2	419529	7	NULL	NULL	0	NULL	internal ward	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A female patient was taken to the internal ward with a tentative diagnosis of recurrent syncope .
	manualset3
212787	3	419529	7	NULL	NULL	0	NULL	tentative diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A female patient was taken to the internal ward with a tentative diagnosis of recurrent syncope .
	manualset3
212788	4	419529	7	NULL	NULL	0	NULL	recurrent syncope	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A female patient was taken to the internal ward with a tentative diagnosis of recurrent syncope .
	manualset3
212805	1	419530	7	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to judge the effect of anthocyanosides and vitamine E ( Difrarel E ) on refraction , visual acuity and eye-fundus , we treated 36 patients with this speciality in progressive myopia .
	manualset3
212806	2	419530	7	NULL	NULL	0	NULL	anthocyanosides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to judge the effect of anthocyanosides and vitamine E ( Difrarel E ) on refraction , visual acuity and eye-fundus , we treated 36 patients with this speciality in progressive myopia .
	manualset3
212807	3	419530	7	NULL	NULL	0	NULL	vitamine E	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to judge the effect of anthocyanosides and vitamine E ( Difrarel E ) on refraction , visual acuity and eye-fundus , we treated 36 patients with this speciality in progressive myopia .
	manualset3
212808	4	419530	7	NULL	NULL	0	NULL	Difrarel E	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to judge the effect of anthocyanosides and vitamine E ( Difrarel E ) on refraction , visual acuity and eye-fundus , we treated 36 patients with this speciality in progressive myopia .
	manualset3
212809	5	419530	7	NULL	NULL	0	NULL	refraction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to judge the effect of anthocyanosides and vitamine E ( Difrarel E ) on refraction , visual acuity and eye-fundus , we treated 36 patients with this speciality in progressive myopia .
	manualset3
212810	6	419530	7	NULL	NULL	0	NULL	visual acuity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to judge the effect of anthocyanosides and vitamine E ( Difrarel E ) on refraction , visual acuity and eye-fundus , we treated 36 patients with this speciality in progressive myopia .
	manualset3
212811	7	419530	7	NULL	NULL	0	NULL	eye-fundus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to judge the effect of anthocyanosides and vitamine E ( Difrarel E ) on refraction , visual acuity and eye-fundus , we treated 36 patients with this speciality in progressive myopia .
	manualset3
212812	8	419530	7	NULL	NULL	0	NULL	36 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to judge the effect of anthocyanosides and vitamine E ( Difrarel E ) on refraction , visual acuity and eye-fundus , we treated 36 patients with this speciality in progressive myopia .
	manualset3
212813	9	419530	7	NULL	NULL	0	NULL	speciality	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to judge the effect of anthocyanosides and vitamine E ( Difrarel E ) on refraction , visual acuity and eye-fundus , we treated 36 patients with this speciality in progressive myopia .
	manualset3
212814	10	419530	7	NULL	NULL	0	NULL	progressive myopia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In order to judge the effect of anthocyanosides and vitamine E ( Difrarel E ) on refraction , visual acuity and eye-fundus , we treated 36 patients with this speciality in progressive myopia .
	manualset3
212961	1	419531	7	NULL	NULL	0	NULL	problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There are problems associated with the use of acute care diagnosis-related groups for prospective payment for rehabilitation medicine services .
	manualset3
212962	2	419531	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There are problems associated with the use of acute care diagnosis-related groups for prospective payment for rehabilitation medicine services .
	manualset3
212963	3	419531	7	NULL	NULL	NULL	NULL	acute care diagnosis-related groups	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There are problems associated with the use of acute care diagnosis-related groups for prospective payment for rehabilitation medicine services .
	manualset3
212964	4	419531	7	NULL	NULL	0	NULL	prospective payment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There are problems associated with the use of acute care diagnosis-related groups for prospective payment for rehabilitation medicine services .
	manualset3
212965	5	419531	7	NULL	NULL	0	NULL	rehabilitation medicine services	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	There are problems associated with the use of acute care diagnosis-related groups for prospective payment for rehabilitation medicine services .
	manualset3
212966	1	419532	7	NULL	NULL	NULL	NULL	washout	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After washout of oxo-M , subsequent exposure to Ca2 + evoked reproducible increases in ( Ca2 + ) i. Application of oxo-M plus Ca2 + had little effect on the increases in ( Ca2 + ) i , indicating that in SH-SY5Y cells , agonist-dependent pathways contribute little to Ca2 + entry following store depletion .
	manualset3
212967	2	419532	7	NULL	NULL	0	NULL	oxo-M	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After washout of oxo-M , subsequent exposure to Ca2 + evoked reproducible increases in ( Ca2 + ) i. Application of oxo-M plus Ca2 + had little effect on the increases in ( Ca2 + ) i , indicating that in SH-SY5Y cells , agonist-dependent pathways contribute little to Ca2 + entry following store depletion .
	manualset3
212968	3	419532	7	NULL	NULL	0	NULL	 exposure 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After washout of oxo-M , subsequent exposure to Ca2 + evoked reproducible increases in ( Ca2 + ) i. Application of oxo-M plus Ca2 + had little effect on the increases in ( Ca2 + ) i , indicating that in SH-SY5Y cells , agonist-dependent pathways contribute little to Ca2 + entry following store depletion .
	manualset3
212969	4	419532	7	NULL	NULL	NULL	NULL	Ca2 + evoked reproducible increases	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After washout of oxo-M , subsequent exposure to Ca2 + evoked reproducible increases in ( Ca2 + ) i. Application of oxo-M plus Ca2 + had little effect on the increases in ( Ca2 + ) i , indicating that in SH-SY5Y cells , agonist-dependent pathways contribute little to Ca2 + entry following store depletion .
	manualset3
212970	5	419532	7	NULL	NULL	0	NULL	( Ca2 + ) i	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After washout of oxo-M , subsequent exposure to Ca2 + evoked reproducible increases in ( Ca2 + ) i. Application of oxo-M plus Ca2 + had little effect on the increases in ( Ca2 + ) i , indicating that in SH-SY5Y cells , agonist-dependent pathways contribute little to Ca2 + entry following store depletion .
	manualset3
212971	6	419532	7	NULL	NULL	0	NULL	Application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After washout of oxo-M , subsequent exposure to Ca2 + evoked reproducible increases in ( Ca2 + ) i. Application of oxo-M plus Ca2 + had little effect on the increases in ( Ca2 + ) i , indicating that in SH-SY5Y cells , agonist-dependent pathways contribute little to Ca2 + entry following store depletion .
	manualset3
212972	7	419532	7	NULL	NULL	0	NULL	oxo-M plus Ca2 +	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After washout of oxo-M , subsequent exposure to Ca2 + evoked reproducible increases in ( Ca2 + ) i. Application of oxo-M plus Ca2 + had little effect on the increases in ( Ca2 + ) i , indicating that in SH-SY5Y cells , agonist-dependent pathways contribute little to Ca2 + entry following store depletion .
	manualset3
212974	8	419532	7	NULL	NULL	0	NULL	 effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After washout of oxo-M , subsequent exposure to Ca2 + evoked reproducible increases in ( Ca2 + ) i. Application of oxo-M plus Ca2 + had little effect on the increases in ( Ca2 + ) i , indicating that in SH-SY5Y cells , agonist-dependent pathways contribute little to Ca2 + entry following store depletion .
	manualset3
212976	9	419532	7	NULL	NULL	0	NULL	 increases	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After washout of oxo-M , subsequent exposure to Ca2 + evoked reproducible increases in ( Ca2 + ) i. Application of oxo-M plus Ca2 + had little effect on the increases in ( Ca2 + ) i , indicating that in SH-SY5Y cells , agonist-dependent pathways contribute little to Ca2 + entry following store depletion .
	manualset3
212977	10	419532	7	NULL	NULL	0	NULL	( Ca2 + ) i	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After washout of oxo-M , subsequent exposure to Ca2 + evoked reproducible increases in ( Ca2 + ) i. Application of oxo-M plus Ca2 + had little effect on the increases in ( Ca2 + ) i , indicating that in SH-SY5Y cells , agonist-dependent pathways contribute little to Ca2 + entry following store depletion .
	manualset3
212979	11	419532	7	NULL	NULL	0	NULL	SH-SY5Y cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	After washout of oxo-M , subsequent exposure to Ca2 + evoked reproducible increases in ( Ca2 + ) i. Application of oxo-M plus Ca2 + had little effect on the increases in ( Ca2 + ) i , indicating that in SH-SY5Y cells , agonist-dependent pathways contribute little to Ca2 + entry following store depletion .
	manualset3
212981	12	419532	7	NULL	NULL	0	NULL	agonist-dependent pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After washout of oxo-M , subsequent exposure to Ca2 + evoked reproducible increases in ( Ca2 + ) i. Application of oxo-M plus Ca2 + had little effect on the increases in ( Ca2 + ) i , indicating that in SH-SY5Y cells , agonist-dependent pathways contribute little to Ca2 + entry following store depletion .
	manualset3
212984	13	419532	7	NULL	NULL	0	NULL	 Ca2 + entry	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After washout of oxo-M , subsequent exposure to Ca2 + evoked reproducible increases in ( Ca2 + ) i. Application of oxo-M plus Ca2 + had little effect on the increases in ( Ca2 + ) i , indicating that in SH-SY5Y cells , agonist-dependent pathways contribute little to Ca2 + entry following store depletion .
	manualset3
212985	14	419532	7	NULL	NULL	0	NULL	store depletion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After washout of oxo-M , subsequent exposure to Ca2 + evoked reproducible increases in ( Ca2 + ) i. Application of oxo-M plus Ca2 + had little effect on the increases in ( Ca2 + ) i , indicating that in SH-SY5Y cells , agonist-dependent pathways contribute little to Ca2 + entry following store depletion .
	manualset3
213087	1	419533	7	NULL	NULL	0	NULL	2 2 layer-buckled manganese oxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A 2 2 layer-buckled manganese oxide , K ( 0.66 ) Mn ( 2 ) O ( 4 ) 0.28 H ( 2 ) O ( I ) , has been synthesized under high pressure and retained at ambient pressure ; it is metastable and will finally transform to a 2 1 layer-buckled K ( 0.99 ) Mn ( 3 ) O ( 6 ) 1.25 H ( 2 ) O ( II ) in 1 year .
	manualset3
213088	2	419533	7	NULL	NULL	0	NULL	K ( 0.66 ) Mn ( 2 ) O ( 4 ) 0.28 H ( 2 ) O ( I )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A 2 2 layer-buckled manganese oxide , K ( 0.66 ) Mn ( 2 ) O ( 4 ) 0.28 H ( 2 ) O ( I ) , has been synthesized under high pressure and retained at ambient pressure ; it is metastable and will finally transform to a 2 1 layer-buckled K ( 0.99 ) Mn ( 3 ) O ( 6 ) 1.25 H ( 2 ) O ( II ) in 1 year .
	manualset3
213089	3	419533	7	NULL	NULL	0	NULL	high pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A 2 2 layer-buckled manganese oxide , K ( 0.66 ) Mn ( 2 ) O ( 4 ) 0.28 H ( 2 ) O ( I ) , has been synthesized under high pressure and retained at ambient pressure ; it is metastable and will finally transform to a 2 1 layer-buckled K ( 0.99 ) Mn ( 3 ) O ( 6 ) 1.25 H ( 2 ) O ( II ) in 1 year .
	manualset3
213090	4	419533	7	NULL	NULL	0	NULL	ambient pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A 2 2 layer-buckled manganese oxide , K ( 0.66 ) Mn ( 2 ) O ( 4 ) 0.28 H ( 2 ) O ( I ) , has been synthesized under high pressure and retained at ambient pressure ; it is metastable and will finally transform to a 2 1 layer-buckled K ( 0.99 ) Mn ( 3 ) O ( 6 ) 1.25 H ( 2 ) O ( II ) in 1 year .
	manualset3
213091	5	419533	7	NULL	NULL	0	NULL	metastable 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A 2 2 layer-buckled manganese oxide , K ( 0.66 ) Mn ( 2 ) O ( 4 ) 0.28 H ( 2 ) O ( I ) , has been synthesized under high pressure and retained at ambient pressure ; it is metastable and will finally transform to a 2 1 layer-buckled K ( 0.99 ) Mn ( 3 ) O ( 6 ) 1.25 H ( 2 ) O ( II ) in 1 year .
	manualset3
213092	6	419533	7	NULL	NULL	0	NULL	2 1 layer-buckled K ( 0.99 ) Mn ( 3 ) O ( 6 ) 1.25 H ( 2 ) O ( II ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A 2 2 layer-buckled manganese oxide , K ( 0.66 ) Mn ( 2 ) O ( 4 ) 0.28 H ( 2 ) O ( I ) , has been synthesized under high pressure and retained at ambient pressure ; it is metastable and will finally transform to a 2 1 layer-buckled K ( 0.99 ) Mn ( 3 ) O ( 6 ) 1.25 H ( 2 ) O ( II ) in 1 year .
	manualset3
213093	7	419533	7	NULL	NULL	0	NULL	1 year	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A 2 2 layer-buckled manganese oxide , K ( 0.66 ) Mn ( 2 ) O ( 4 ) 0.28 H ( 2 ) O ( I ) , has been synthesized under high pressure and retained at ambient pressure ; it is metastable and will finally transform to a 2 1 layer-buckled K ( 0.99 ) Mn ( 3 ) O ( 6 ) 1.25 H ( 2 ) O ( II ) in 1 year .
	manualset3
213094	1	419534	7	NULL	NULL	0	NULL	case-control study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case-control study for CNV occurrence , 327 highly myopic Japanese patients were enrolled .
	manualset3
213095	2	419534	7	NULL	NULL	0	NULL	CNV occurrence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case-control study for CNV occurrence , 327 highly myopic Japanese patients were enrolled .
	manualset3
213096	3	419534	7	NULL	NULL	0	NULL	327 highly myopic Japanese patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case-control study for CNV occurrence , 327 highly myopic Japanese patients were enrolled .
	manualset3
213097	1	419535	7	NULL	NULL	0	NULL	complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were some complications related to surgical error or lack of strict compliance with the qualification criteria .
	manualset3
213098	2	419535	7	NULL	NULL	0	NULL	surgical error 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There were some complications related to surgical error or lack of strict compliance with the qualification criteria .
	manualset3
213099	3	419535	7	NULL	NULL	0	NULL	lack	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There were some complications related to surgical error or lack of strict compliance with the qualification criteria .
	manualset3
213100	4	419535	7	NULL	NULL	0	NULL	strict compliance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There were some complications related to surgical error or lack of strict compliance with the qualification criteria .
	manualset3
213101	5	419535	7	NULL	NULL	0	NULL	qualification criteria	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There were some complications related to surgical error or lack of strict compliance with the qualification criteria .
	manualset3
213102	1	419536	7	NULL	NULL	0	NULL	stacks	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	These stacks thus function as independent mating groups in which individuals may reproduce consecutively as male and female over a short time period , a pattern explained by sperm storage capacity .
	manualset3
213103	2	419536	7	NULL	NULL	0	NULL	 independent mating groups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These stacks thus function as independent mating groups in which individuals may reproduce consecutively as male and female over a short time period , a pattern explained by sperm storage capacity .
	manualset3
213104	3	419536	7	NULL	NULL	0	NULL	 individuals 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	These stacks thus function as independent mating groups in which individuals may reproduce consecutively as male and female over a short time period , a pattern explained by sperm storage capacity .
	manualset3
213105	4	419536	7	NULL	NULL	0	NULL	male	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	These stacks thus function as independent mating groups in which individuals may reproduce consecutively as male and female over a short time period , a pattern explained by sperm storage capacity .
	manualset3
213106	5	419536	7	NULL	NULL	0	NULL	female	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	These stacks thus function as independent mating groups in which individuals may reproduce consecutively as male and female over a short time period , a pattern explained by sperm storage capacity .
	manualset3
213107	6	419536	7	NULL	NULL	0	NULL	short time period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	These stacks thus function as independent mating groups in which individuals may reproduce consecutively as male and female over a short time period , a pattern explained by sperm storage capacity .
	manualset3
213108	7	419536	7	NULL	NULL	0	NULL	pattern	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These stacks thus function as independent mating groups in which individuals may reproduce consecutively as male and female over a short time period , a pattern explained by sperm storage capacity .
	manualset3
213109	8	419536	7	NULL	NULL	0	NULL	sperm storage capacity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These stacks thus function as independent mating groups in which individuals may reproduce consecutively as male and female over a short time period , a pattern explained by sperm storage capacity .
	manualset3
213110	1	419537	7	NULL	NULL	0	NULL	inflammation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	During inflammation , MMP-2 expression was increased in epithelial cells as well as in the infiltrating immune cells .
	manualset3
213111	2	419537	7	NULL	NULL	0	NULL	MMP-2 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	During inflammation , MMP-2 expression was increased in epithelial cells as well as in the infiltrating immune cells .
	manualset3
213112	3	419537	7	NULL	NULL	0	NULL	epithelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	During inflammation , MMP-2 expression was increased in epithelial cells as well as in the infiltrating immune cells .
	manualset3
213113	4	419537	7	NULL	NULL	0	NULL	infiltrating immune cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	During inflammation , MMP-2 expression was increased in epithelial cells as well as in the infiltrating immune cells .
	manualset3
213114	1	419538	7	NULL	NULL	0	NULL	Natural therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Natural therapy of poliomyelitis and of its preliminary states ) .
	manualset3
213115	2	419538	7	NULL	NULL	0	NULL	 poliomyelitis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Natural therapy of poliomyelitis and of its preliminary states ) .
	manualset3
213116	3	419538	7	NULL	NULL	0	NULL	preliminary states	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Natural therapy of poliomyelitis and of its preliminary states ) .
	manualset3
213117	1	419539	7	NULL	NULL	0	NULL	Repercussions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Repercussions of triamcinolone on physiologic nyctohemeral biorhythm of free plasmatic 11-oxycorticosteroids of man ) .
	manualset3
213118	2	419539	7	NULL	NULL	0	NULL	triamcinolone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Repercussions of triamcinolone on physiologic nyctohemeral biorhythm of free plasmatic 11-oxycorticosteroids of man ) .
	manualset3
213119	3	419539	7	NULL	NULL	0	NULL	physiologic nyctohemeral biorhythm	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Repercussions of triamcinolone on physiologic nyctohemeral biorhythm of free plasmatic 11-oxycorticosteroids of man ) .
	manualset3
213120	4	419539	7	NULL	NULL	NULL	NULL	free plasmatic 11-oxycorticosteroids	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Repercussions of triamcinolone on physiologic nyctohemeral biorhythm of free plasmatic 11-oxycorticosteroids of man ) .
	manualset3
213121	5	419539	7	NULL	NULL	0	NULL	man	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( Repercussions of triamcinolone on physiologic nyctohemeral biorhythm of free plasmatic 11-oxycorticosteroids of man ) .
	manualset3
213122	1	419540	7	NULL	NULL	0	NULL	Achilles ' heel	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The other Achilles ' heel of BCR-ABL1 .
	manualset3
213123	2	419540	7	NULL	NULL	0	NULL	BCR-ABL1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The other Achilles ' heel of BCR-ABL1 .
	manualset3
213177	1	419541	7	NULL	NULL	0	NULL	Concentrated multidisciplinary treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrated multidisciplinary treatment reduces post treatment morbidity by shortening recovery and rehabilitation time .
	manualset3
213178	2	419541	7	NULL	NULL	0	NULL	post treatment morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrated multidisciplinary treatment reduces post treatment morbidity by shortening recovery and rehabilitation time .
	manualset3
213179	3	419541	7	NULL	NULL	0	NULL	shortening recovery	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrated multidisciplinary treatment reduces post treatment morbidity by shortening recovery and rehabilitation time .
	manualset3
213180	4	419541	7	NULL	NULL	0	NULL	rehabilitation time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrated multidisciplinary treatment reduces post treatment morbidity by shortening recovery and rehabilitation time .
	manualset3
213181	1	419542	7	NULL	NULL	0	NULL	no task-group	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although no task-group of MU was found among the muscles , it appeared that a higher proportion of fast MU was recruited within the muscles of the first group during the upper part of the PBGS .
	manualset3
213182	2	419542	7	NULL	NULL	0	NULL	MU	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although no task-group of MU was found among the muscles , it appeared that a higher proportion of fast MU was recruited within the muscles of the first group during the upper part of the PBGS .
	manualset3
213183	3	419542	7	NULL	NULL	0	NULL	muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although no task-group of MU was found among the muscles , it appeared that a higher proportion of fast MU was recruited within the muscles of the first group during the upper part of the PBGS .
	manualset3
213184	4	419542	7	NULL	NULL	0	NULL	higher proportion	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although no task-group of MU was found among the muscles , it appeared that a higher proportion of fast MU was recruited within the muscles of the first group during the upper part of the PBGS .
	manualset3
213185	5	419542	7	NULL	NULL	0	NULL	fast MU	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although no task-group of MU was found among the muscles , it appeared that a higher proportion of fast MU was recruited within the muscles of the first group during the upper part of the PBGS .
	manualset3
213186	6	419542	7	NULL	NULL	0	NULL	muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although no task-group of MU was found among the muscles , it appeared that a higher proportion of fast MU was recruited within the muscles of the first group during the upper part of the PBGS .
	manualset3
213187	7	419542	7	NULL	NULL	0	NULL	first group	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although no task-group of MU was found among the muscles , it appeared that a higher proportion of fast MU was recruited within the muscles of the first group during the upper part of the PBGS .
	manualset3
213188	8	419542	7	NULL	NULL	0	NULL	upper part	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although no task-group of MU was found among the muscles , it appeared that a higher proportion of fast MU was recruited within the muscles of the first group during the upper part of the PBGS .
	manualset3
213189	9	419542	7	NULL	NULL	0	NULL	PBGS	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although no task-group of MU was found among the muscles , it appeared that a higher proportion of fast MU was recruited within the muscles of the first group during the upper part of the PBGS .
	manualset3
213190	1	419543	7	NULL	NULL	0	NULL	Retention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Retention of lithium induced by ethanol appeared to be responsible for the potentiation of lithium toxicity .
	manualset3
213191	2	419543	7	NULL	NULL	0	NULL	lithium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Retention of lithium induced by ethanol appeared to be responsible for the potentiation of lithium toxicity .
	manualset3
213192	3	419543	7	NULL	NULL	0	NULL	ethanol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Retention of lithium induced by ethanol appeared to be responsible for the potentiation of lithium toxicity .
	manualset3
213193	4	419543	7	NULL	NULL	0	NULL	potentiation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Retention of lithium induced by ethanol appeared to be responsible for the potentiation of lithium toxicity .
	manualset3
213194	5	419543	7	NULL	NULL	0	NULL	lithium toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Retention of lithium induced by ethanol appeared to be responsible for the potentiation of lithium toxicity .
	manualset3
213242	1	419544	7	NULL	NULL	0	NULL	gene expression grade index ( GGI )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A gene expression grade index ( GGI ) was developed that challenges the existence and clinical relevance of an intermediate grade 2 classification .
	manualset3
213246	2	419544	7	NULL	NULL	0	NULL	 existence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A gene expression grade index ( GGI ) was developed that challenges the existence and clinical relevance of an intermediate grade 2 classification .
	manualset3
213250	3	419544	7	NULL	NULL	0	NULL	clinical relevance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A gene expression grade index ( GGI ) was developed that challenges the existence and clinical relevance of an intermediate grade 2 classification .
	manualset3
213253	4	419544	7	NULL	NULL	0	NULL	intermediate grade 2 classification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A gene expression grade index ( GGI ) was developed that challenges the existence and clinical relevance of an intermediate grade 2 classification .
	manualset3
213265	1	419545	7	NULL	NULL	NULL	NULL	Integrin adhesion	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Integrin adhesion and force coupling are independently regulated by localized PtdIns ( 4 , 5 ) 2 synthesis .
	manualset3
213266	2	419545	7	NULL	NULL	0	NULL	 force coupling 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrin adhesion and force coupling are independently regulated by localized PtdIns ( 4 , 5 ) 2 synthesis .
	manualset3
213267	3	419545	7	NULL	NULL	0	NULL	PtdIns ( 4 , 5 ) 2 synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrin adhesion and force coupling are independently regulated by localized PtdIns ( 4 , 5 ) 2 synthesis .
	manualset3
213268	1	419546	7	NULL	NULL	0	NULL	Human plasma TPO concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Human plasma TPO concentration correlated with the platelet counts .
	manualset3
213269	2	419546	7	NULL	NULL	0	NULL	platelet counts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Human plasma TPO concentration correlated with the platelet counts .
	manualset3
213270	1	419547	7	NULL	NULL	0	NULL	IL-33-induced Th2 response 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , IL-33-induced Th2 response was enhanced in SIGIRR-deficient mice compared with that in wild-type control mice , suggesting a negative regulatory role of SIGIRR in IL-33 / ST2 signaling in vivo .
	manualset3
213271	2	419547	7	NULL	NULL	0	NULL	SIGIRR-deficient mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , IL-33-induced Th2 response was enhanced in SIGIRR-deficient mice compared with that in wild-type control mice , suggesting a negative regulatory role of SIGIRR in IL-33 / ST2 signaling in vivo .
	manualset3
213272	3	419547	7	NULL	NULL	0	NULL	wild-type control mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , IL-33-induced Th2 response was enhanced in SIGIRR-deficient mice compared with that in wild-type control mice , suggesting a negative regulatory role of SIGIRR in IL-33 / ST2 signaling in vivo .
	manualset3
213273	4	419547	7	NULL	NULL	0	NULL	negative regulatory role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , IL-33-induced Th2 response was enhanced in SIGIRR-deficient mice compared with that in wild-type control mice , suggesting a negative regulatory role of SIGIRR in IL-33 / ST2 signaling in vivo .
	manualset3
213334	6	419547	7	NULL	NULL	NULL	NULL	IL-33 / ST2 signaling	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , IL-33-induced Th2 response was enhanced in SIGIRR-deficient mice compared with that in wild-type control mice , suggesting a negative regulatory role of SIGIRR in IL-33 / ST2 signaling in vivo .
	manualset3
214849	5	419547	7	NULL	NULL	0	NULL	 SIGIRR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , IL-33-induced Th2 response was enhanced in SIGIRR-deficient mice compared with that in wild-type control mice , suggesting a negative regulatory role of SIGIRR in IL-33 / ST2 signaling in vivo .
	manualset3
213335	1	419548	7	NULL	NULL	0	NULL	 vaccines	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Although no vaccines or antiviral drugs for MARV are currently available , remarkable progress has been made over the last few years in developing potential countermeasures against MARV in nonhuman primate models .
	manualset3
213336	2	419548	7	NULL	NULL	0	NULL	antiviral drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Although no vaccines or antiviral drugs for MARV are currently available , remarkable progress has been made over the last few years in developing potential countermeasures against MARV in nonhuman primate models .
	manualset3
213337	3	419548	7	NULL	NULL	0	NULL	MARV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although no vaccines or antiviral drugs for MARV are currently available , remarkable progress has been made over the last few years in developing potential countermeasures against MARV in nonhuman primate models .
	manualset3
213338	4	419548	7	NULL	NULL	0	NULL	progress	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although no vaccines or antiviral drugs for MARV are currently available , remarkable progress has been made over the last few years in developing potential countermeasures against MARV in nonhuman primate models .
	manualset3
213339	5	419548	7	NULL	NULL	0	NULL	few years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Although no vaccines or antiviral drugs for MARV are currently available , remarkable progress has been made over the last few years in developing potential countermeasures against MARV in nonhuman primate models .
	manualset3
213340	6	419548	7	NULL	NULL	0	NULL	potential countermeasures 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although no vaccines or antiviral drugs for MARV are currently available , remarkable progress has been made over the last few years in developing potential countermeasures against MARV in nonhuman primate models .
	manualset3
213341	7	419548	7	NULL	NULL	0	NULL	MARV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although no vaccines or antiviral drugs for MARV are currently available , remarkable progress has been made over the last few years in developing potential countermeasures against MARV in nonhuman primate models .
	manualset3
213342	8	419548	7	NULL	NULL	0	NULL	nonhuman primate models	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although no vaccines or antiviral drugs for MARV are currently available , remarkable progress has been made over the last few years in developing potential countermeasures against MARV in nonhuman primate models .
	manualset3
213343	1	419549	7	NULL	NULL	0	NULL	unobtrusive system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	An unobtrusive system , which provided corrective feedback ( vibratory stimulation ) for an incorrect direction , was used to help a woman with deafness and profound intellectual and visual disabilities during her indoor travel .
	manualset3
213344	2	419549	7	NULL	NULL	0	NULL	corrective feedback	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An unobtrusive system , which provided corrective feedback ( vibratory stimulation ) for an incorrect direction , was used to help a woman with deafness and profound intellectual and visual disabilities during her indoor travel .
	manualset3
213345	3	419549	7	NULL	NULL	0	NULL	vibratory stimulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An unobtrusive system , which provided corrective feedback ( vibratory stimulation ) for an incorrect direction , was used to help a woman with deafness and profound intellectual and visual disabilities during her indoor travel .
	manualset3
213346	4	419549	7	NULL	NULL	0	NULL	incorrect direction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An unobtrusive system , which provided corrective feedback ( vibratory stimulation ) for an incorrect direction , was used to help a woman with deafness and profound intellectual and visual disabilities during her indoor travel .
	manualset3
213347	5	419549	7	NULL	NULL	0	NULL	woman	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	An unobtrusive system , which provided corrective feedback ( vibratory stimulation ) for an incorrect direction , was used to help a woman with deafness and profound intellectual and visual disabilities during her indoor travel .
	manualset3
213348	6	419549	7	NULL	NULL	0	NULL	deafness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An unobtrusive system , which provided corrective feedback ( vibratory stimulation ) for an incorrect direction , was used to help a woman with deafness and profound intellectual and visual disabilities during her indoor travel .
	manualset3
213349	7	419549	7	NULL	NULL	0	NULL	intellectual disabilities	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An unobtrusive system , which provided corrective feedback ( vibratory stimulation ) for an incorrect direction , was used to help a woman with deafness and profound intellectual and visual disabilities during her indoor travel .
	manualset3
213350	8	419549	7	NULL	NULL	0	NULL	visual disabilities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An unobtrusive system , which provided corrective feedback ( vibratory stimulation ) for an incorrect direction , was used to help a woman with deafness and profound intellectual and visual disabilities during her indoor travel .
	manualset3
213351	9	419549	7	NULL	NULL	0	NULL	indoor travel	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An unobtrusive system , which provided corrective feedback ( vibratory stimulation ) for an incorrect direction , was used to help a woman with deafness and profound intellectual and visual disabilities during her indoor travel .
	manualset3
213352	1	419550	7	NULL	NULL	0	NULL	 changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , changes in daily illumination serve as the time indicator for circadian rhythms of cell proliferation , but not for ultradian oscillations of mitotic activity .
	manualset3
213353	2	419550	7	NULL	NULL	0	NULL	daily illumination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , changes in daily illumination serve as the time indicator for circadian rhythms of cell proliferation , but not for ultradian oscillations of mitotic activity .
	manualset3
213354	3	419550	7	NULL	NULL	0	NULL	time indicator 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , changes in daily illumination serve as the time indicator for circadian rhythms of cell proliferation , but not for ultradian oscillations of mitotic activity .
	manualset3
213355	4	419550	7	NULL	NULL	0	NULL	 circadian rhythms 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , changes in daily illumination serve as the time indicator for circadian rhythms of cell proliferation , but not for ultradian oscillations of mitotic activity .
	manualset3
213356	5	419550	7	NULL	NULL	0	NULL	cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , changes in daily illumination serve as the time indicator for circadian rhythms of cell proliferation , but not for ultradian oscillations of mitotic activity .
	manualset3
213357	6	419550	7	NULL	NULL	0	NULL	ultradian oscillations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , changes in daily illumination serve as the time indicator for circadian rhythms of cell proliferation , but not for ultradian oscillations of mitotic activity .
	manualset3
213358	7	419550	7	NULL	NULL	0	NULL	mitotic activity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , changes in daily illumination serve as the time indicator for circadian rhythms of cell proliferation , but not for ultradian oscillations of mitotic activity .
	manualset3
213359	1	419551	7	NULL	NULL	0	NULL	Pretreatment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with selective PKC and inhibitors blocked CLS formation .
	manualset3
213360	2	419551	7	NULL	NULL	0	NULL	 selective PKC	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with selective PKC and inhibitors blocked CLS formation .
	manualset3
213361	3	419551	7	NULL	NULL	0	NULL	inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with selective PKC and inhibitors blocked CLS formation .
	manualset3
213362	4	419551	7	NULL	NULL	0	NULL	CLS formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with selective PKC and inhibitors blocked CLS formation .
	manualset3
213363	1	419552	7	NULL	NULL	0	NULL	Lysosomal activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysosomal activity in aging rat liver : I. Variation in enzyme activity within the liver lobule .
	manualset3
213364	2	419552	7	NULL	NULL	0	NULL	aging rat liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysosomal activity in aging rat liver : I. Variation in enzyme activity within the liver lobule .
	manualset3
213365	3	419552	7	NULL	NULL	0	NULL	Variation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysosomal activity in aging rat liver : I. Variation in enzyme activity within the liver lobule .
	manualset3
213366	4	419552	7	NULL	NULL	0	NULL	enzyme activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysosomal activity in aging rat liver : I. Variation in enzyme activity within the liver lobule .
	manualset3
213367	5	419552	7	NULL	NULL	0	NULL	liver lobule	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Lysosomal activity in aging rat liver : I. Variation in enzyme activity within the liver lobule .
	manualset3
213368	1	419553	7	NULL	NULL	0	NULL	Registered retirement savings plans	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Registered retirement savings plans : now is the time to decide .
	manualset3
213369	2	419553	7	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Registered retirement savings plans : now is the time to decide .
	manualset3
213370	1	419554	7	NULL	NULL	0	NULL	Salt	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Salt , palatability and future health .
	manualset3
213371	2	419554	7	NULL	NULL	0	NULL	palatability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Salt , palatability and future health .
	manualset3
213372	3	419554	7	NULL	NULL	0	NULL	future health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Salt , palatability and future health .
	manualset3
213373	1	419555	7	NULL	NULL	0	NULL	Thirty percent	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty percent of cases were caused by coinfection with hepatitis B virus and hepatitis delta virus or by infection with hepatitis delta virus superimposed on carriers of chronic HBsAg .
	manualset3
213374	2	419555	7	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty percent of cases were caused by coinfection with hepatitis B virus and hepatitis delta virus or by infection with hepatitis delta virus superimposed on carriers of chronic HBsAg .
	manualset3
213375	3	419555	7	NULL	NULL	NULL	NULL	coinfection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Thirty percent of cases were caused by coinfection with hepatitis B virus and hepatitis delta virus or by infection with hepatitis delta virus superimposed on carriers of chronic HBsAg .
	manualset3
213376	4	419555	7	NULL	NULL	0	NULL	hepatitis B virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty percent of cases were caused by coinfection with hepatitis B virus and hepatitis delta virus or by infection with hepatitis delta virus superimposed on carriers of chronic HBsAg .
	manualset3
213377	5	419555	7	NULL	NULL	0	NULL	hepatitis delta virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty percent of cases were caused by coinfection with hepatitis B virus and hepatitis delta virus or by infection with hepatitis delta virus superimposed on carriers of chronic HBsAg .
	manualset3
213378	6	419555	7	NULL	NULL	0	NULL	infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty percent of cases were caused by coinfection with hepatitis B virus and hepatitis delta virus or by infection with hepatitis delta virus superimposed on carriers of chronic HBsAg .
	manualset3
213379	7	419555	7	NULL	NULL	0	NULL	hepatitis delta virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty percent of cases were caused by coinfection with hepatitis B virus and hepatitis delta virus or by infection with hepatitis delta virus superimposed on carriers of chronic HBsAg .
	manualset3
213380	8	419555	7	NULL	NULL	NULL	NULL	carriers	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Thirty percent of cases were caused by coinfection with hepatitis B virus and hepatitis delta virus or by infection with hepatitis delta virus superimposed on carriers of chronic HBsAg .
	manualset3
213381	9	419555	7	NULL	NULL	0	NULL	chronic HBsAg	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty percent of cases were caused by coinfection with hepatitis B virus and hepatitis delta virus or by infection with hepatitis delta virus superimposed on carriers of chronic HBsAg .
	manualset3
213382	1	419556	7	NULL	NULL	0	NULL	Cytotoxic action 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cytotoxic action of immune lymphocytes on `` adherent '' cells ( macrophages ) of autologous system lymph nodes during delayed hypersensitivity ) .
	manualset3
213383	2	419556	7	NULL	NULL	0	NULL	immune lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cytotoxic action of immune lymphocytes on `` adherent '' cells ( macrophages ) of autologous system lymph nodes during delayed hypersensitivity ) .
	manualset3
213384	3	419556	7	NULL	NULL	0	NULL	`` adherent '' cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cytotoxic action of immune lymphocytes on `` adherent '' cells ( macrophages ) of autologous system lymph nodes during delayed hypersensitivity ) .
	manualset3
213385	4	419556	7	NULL	NULL	0	NULL	macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cytotoxic action of immune lymphocytes on `` adherent '' cells ( macrophages ) of autologous system lymph nodes during delayed hypersensitivity ) .
	manualset3
213386	5	419556	7	NULL	NULL	0	NULL	autologous system lymph nodes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cytotoxic action of immune lymphocytes on `` adherent '' cells ( macrophages ) of autologous system lymph nodes during delayed hypersensitivity ) .
	manualset3
213387	6	419556	7	NULL	NULL	0	NULL	delayed hypersensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cytotoxic action of immune lymphocytes on `` adherent '' cells ( macrophages ) of autologous system lymph nodes during delayed hypersensitivity ) .
	manualset3
213388	1	419557	7	NULL	NULL	0	NULL	nonsteroidal anti-inflammatory drugs ( NSAIDs )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Although nonsteroidal anti-inflammatory drugs ( NSAIDs ) provide important control of pain and inflammation , they have been overshadowed by concerns regarding atherothrombotic complications .
	manualset3
213389	2	419557	7	NULL	NULL	0	NULL	 control	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although nonsteroidal anti-inflammatory drugs ( NSAIDs ) provide important control of pain and inflammation , they have been overshadowed by concerns regarding atherothrombotic complications .
	manualset3
213390	3	419557	7	NULL	NULL	0	NULL	pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although nonsteroidal anti-inflammatory drugs ( NSAIDs ) provide important control of pain and inflammation , they have been overshadowed by concerns regarding atherothrombotic complications .
	manualset3
213391	4	419557	7	NULL	NULL	0	NULL	inflammation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although nonsteroidal anti-inflammatory drugs ( NSAIDs ) provide important control of pain and inflammation , they have been overshadowed by concerns regarding atherothrombotic complications .
	manualset3
213392	5	419557	7	NULL	NULL	0	NULL	atherothrombotic complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although nonsteroidal anti-inflammatory drugs ( NSAIDs ) provide important control of pain and inflammation , they have been overshadowed by concerns regarding atherothrombotic complications .
	manualset3
213393	1	419558	7	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors took into account not only anatomical and hemodynamic contraindications for Fontana 's operation , but the latter was not performed when the patient 's status was grave ( severe hypoxemia ) .
	manualset3
213394	2	419558	7	NULL	NULL	0	NULL	anatomical contraindications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors took into account not only anatomical and hemodynamic contraindications for Fontana 's operation , but the latter was not performed when the patient 's status was grave ( severe hypoxemia ) .
	manualset3
213395	3	419558	7	NULL	NULL	0	NULL	hemodynamic contraindications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors took into account not only anatomical and hemodynamic contraindications for Fontana 's operation , but the latter was not performed when the patient 's status was grave ( severe hypoxemia ) .
	manualset3
213396	4	419558	7	NULL	NULL	0	NULL	Fontana 's operation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors took into account not only anatomical and hemodynamic contraindications for Fontana 's operation , but the latter was not performed when the patient 's status was grave ( severe hypoxemia ) .
	manualset3
213397	5	419558	7	NULL	NULL	0	NULL	patient 's status 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors took into account not only anatomical and hemodynamic contraindications for Fontana 's operation , but the latter was not performed when the patient 's status was grave ( severe hypoxemia ) .
	manualset3
213398	6	419558	7	NULL	NULL	0	NULL	grave	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors took into account not only anatomical and hemodynamic contraindications for Fontana 's operation , but the latter was not performed when the patient 's status was grave ( severe hypoxemia ) .
	manualset3
213399	7	419558	7	NULL	NULL	0	NULL	severe hypoxemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors took into account not only anatomical and hemodynamic contraindications for Fontana 's operation , but the latter was not performed when the patient 's status was grave ( severe hypoxemia ) .
	manualset3
213400	1	419559	7	NULL	NULL	NULL	NULL	MSA groups	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Comparing the MSA and PD groups , ( PCr ) was significantly lower in MSA than in PD , whereas cytosolic free ( Mg2 + ) was significantly lower in PD .
	manualset3
213401	2	419559	7	NULL	NULL	0	NULL	PD groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the MSA and PD groups , ( PCr ) was significantly lower in MSA than in PD , whereas cytosolic free ( Mg2 + ) was significantly lower in PD .
	manualset3
213402	3	419559	7	NULL	NULL	0	NULL	 PCr	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the MSA and PD groups , ( PCr ) was significantly lower in MSA than in PD , whereas cytosolic free ( Mg2 + ) was significantly lower in PD .
	manualset3
213403	4	419559	7	NULL	NULL	0	NULL	MSA	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the MSA and PD groups , ( PCr ) was significantly lower in MSA than in PD , whereas cytosolic free ( Mg2 + ) was significantly lower in PD .
	manualset3
213404	5	419559	7	NULL	NULL	0	NULL	PD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the MSA and PD groups , ( PCr ) was significantly lower in MSA than in PD , whereas cytosolic free ( Mg2 + ) was significantly lower in PD .
	manualset3
213405	6	419559	7	NULL	NULL	0	NULL	cytosolic free ( Mg2 + ) 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the MSA and PD groups , ( PCr ) was significantly lower in MSA than in PD , whereas cytosolic free ( Mg2 + ) was significantly lower in PD .
	manualset3
213406	7	419559	7	NULL	NULL	0	NULL	PD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the MSA and PD groups , ( PCr ) was significantly lower in MSA than in PD , whereas cytosolic free ( Mg2 + ) was significantly lower in PD .
	manualset3
213407	1	419560	7	NULL	NULL	0	NULL	Ten cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten cases of SPA were documented by CT scan ( 8 % ) .
	manualset3
213408	2	419560	7	NULL	NULL	0	NULL	SPA	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten cases of SPA were documented by CT scan ( 8 % ) .
	manualset3
213409	3	419560	7	NULL	NULL	0	NULL	CT scan	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten cases of SPA were documented by CT scan ( 8 % ) .
	manualset3
213410	4	419560	7	NULL	NULL	0	NULL	8 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten cases of SPA were documented by CT scan ( 8 % ) .
	manualset3
213411	1	419561	7	NULL	NULL	0	NULL	closer look	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A closer look at the relationship between restrained eating and vegetarianism in college females .
	manualset3
213412	2	419561	7	NULL	NULL	0	NULL	 relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A closer look at the relationship between restrained eating and vegetarianism in college females .
	manualset3
213413	3	419561	7	NULL	NULL	0	NULL	restrained eating	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A closer look at the relationship between restrained eating and vegetarianism in college females .
	manualset3
213414	4	419561	7	NULL	NULL	0	NULL	vegetarianism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A closer look at the relationship between restrained eating and vegetarianism in college females .
	manualset3
213415	5	419561	7	NULL	NULL	0	NULL	college females	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A closer look at the relationship between restrained eating and vegetarianism in college females .
	manualset3
213416	1	419562	7	NULL	NULL	0	NULL	TG11	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	TG11 , 15 and 19 had low spontaneous mutant frequencies which were either unaffected or only marginally increased by treatment with 5-azacytidine .
	manualset3
213417	2	419562	7	NULL	NULL	0	NULL	TG15	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	TG11 , 15 and 19 had low spontaneous mutant frequencies which were either unaffected or only marginally increased by treatment with 5-azacytidine .
	manualset3
213418	3	419562	7	NULL	NULL	0	NULL	TG19	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	TG11 , 15 and 19 had low spontaneous mutant frequencies which were either unaffected or only marginally increased by treatment with 5-azacytidine .
	manualset3
213419	4	419562	7	NULL	NULL	0	NULL	spontaneous mutant frequencies	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	TG11 , 15 and 19 had low spontaneous mutant frequencies which were either unaffected or only marginally increased by treatment with 5-azacytidine .
	manualset3
213420	5	419562	7	NULL	NULL	0	NULL	treatment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	TG11 , 15 and 19 had low spontaneous mutant frequencies which were either unaffected or only marginally increased by treatment with 5-azacytidine .
	manualset3
213421	6	419562	7	NULL	NULL	0	NULL	5-azacytidine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	TG11 , 15 and 19 had low spontaneous mutant frequencies which were either unaffected or only marginally increased by treatment with 5-azacytidine .
	manualset3
213422	1	419563	7	NULL	NULL	0	NULL	Pruritus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pruritus at the site of active acne has not been described before as a complication of acne therapy .
	manualset3
213423	2	419563	7	NULL	NULL	0	NULL	site	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Pruritus at the site of active acne has not been described before as a complication of acne therapy .
	manualset3
213424	3	419563	7	NULL	NULL	0	NULL	active acne 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pruritus at the site of active acne has not been described before as a complication of acne therapy .
	manualset3
213425	4	419563	7	NULL	NULL	0	NULL	complication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pruritus at the site of active acne has not been described before as a complication of acne therapy .
	manualset3
213426	5	419563	7	NULL	NULL	0	NULL	acne therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pruritus at the site of active acne has not been described before as a complication of acne therapy .
	manualset3
213427	1	419564	7	NULL	NULL	0	NULL	Southern transfer	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Southern transfer and genetic analyses of strains carrying a disrupted leu3 allele demonstrated that the cloned gene was LEU3 , as opposed to a suppressor .
	manualset3
213428	2	419564	7	NULL	NULL	0	NULL	genetic analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Southern transfer and genetic analyses of strains carrying a disrupted leu3 allele demonstrated that the cloned gene was LEU3 , as opposed to a suppressor .
	manualset3
213429	3	419564	7	NULL	NULL	0	NULL	strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Southern transfer and genetic analyses of strains carrying a disrupted leu3 allele demonstrated that the cloned gene was LEU3 , as opposed to a suppressor .
	manualset3
213430	4	419564	7	NULL	NULL	0	NULL	leu3 allele	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Southern transfer and genetic analyses of strains carrying a disrupted leu3 allele demonstrated that the cloned gene was LEU3 , as opposed to a suppressor .
	manualset3
213431	5	419564	7	NULL	NULL	0	NULL	cloned gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Southern transfer and genetic analyses of strains carrying a disrupted leu3 allele demonstrated that the cloned gene was LEU3 , as opposed to a suppressor .
	manualset3
213432	6	419564	7	NULL	NULL	0	NULL	LEU3	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Southern transfer and genetic analyses of strains carrying a disrupted leu3 allele demonstrated that the cloned gene was LEU3 , as opposed to a suppressor .
	manualset3
213433	7	419564	7	NULL	NULL	0	NULL	suppressor 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Southern transfer and genetic analyses of strains carrying a disrupted leu3 allele demonstrated that the cloned gene was LEU3 , as opposed to a suppressor .
	manualset3
213434	1	419565	7	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These cases involved 96 law enforcement jurisdictions in 26 different states .
	manualset3
213435	2	419565	7	NULL	NULL	0	NULL	96 law enforcement jurisdictions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These cases involved 96 law enforcement jurisdictions in 26 different states .
	manualset3
213436	3	419565	7	NULL	NULL	0	NULL	26 different states	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	These cases involved 96 law enforcement jurisdictions in 26 different states .
	manualset3
213437	1	419566	7	NULL	NULL	0	NULL	Initial experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial experience with the Forte plate for dorsally displaced distal radius fractures .
	manualset3
213438	2	419566	7	NULL	NULL	0	NULL	Forte plate	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial experience with the Forte plate for dorsally displaced distal radius fractures .
	manualset3
213439	3	419566	7	NULL	NULL	0	NULL	 dorsally displaced distal radius fractures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Initial experience with the Forte plate for dorsally displaced distal radius fractures .
	manualset3
213440	1	419567	7	NULL	NULL	NULL	NULL	priori hypotheses	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although not a priori hypotheses , family history of depression ( adjusted OR = 1.28 , 95 % CI 1.04 , 1.57 ; p = 0.018 ) , and younger maternal age ( adjusted OR per 10-year age increase = 0.62 , 95 % CI 0.47 , 0.82 ; p & lt ; 0.001 ) both showed stronger evidence of association with suspected or definite PLIKS .
	manualset3
213441	2	419567	7	NULL	NULL	0	NULL	family history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although not a priori hypotheses , family history of depression ( adjusted OR = 1.28 , 95 % CI 1.04 , 1.57 ; p = 0.018 ) , and younger maternal age ( adjusted OR per 10-year age increase = 0.62 , 95 % CI 0.47 , 0.82 ; p & lt ; 0.001 ) both showed stronger evidence of association with suspected or definite PLIKS .
	manualset3
213442	3	419567	7	NULL	NULL	0	NULL	depression	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Although not a priori hypotheses , family history of depression ( adjusted OR = 1.28 , 95 % CI 1.04 , 1.57 ; p = 0.018 ) , and younger maternal age ( adjusted OR per 10-year age increase = 0.62 , 95 % CI 0.47 , 0.82 ; p & lt ; 0.001 ) both showed stronger evidence of association with suspected or definite PLIKS .
	manualset3
213443	4	419567	7	NULL	NULL	NULL	NULL	OR = 1.28	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although not a priori hypotheses , family history of depression ( adjusted OR = 1.28 , 95 % CI 1.04 , 1.57 ; p = 0.018 ) , and younger maternal age ( adjusted OR per 10-year age increase = 0.62 , 95 % CI 0.47 , 0.82 ; p & lt ; 0.001 ) both showed stronger evidence of association with suspected or definite PLIKS .
	manualset3
213444	5	419567	7	NULL	NULL	0	NULL	95 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although not a priori hypotheses , family history of depression ( adjusted OR = 1.28 , 95 % CI 1.04 , 1.57 ; p = 0.018 ) , and younger maternal age ( adjusted OR per 10-year age increase = 0.62 , 95 % CI 0.47 , 0.82 ; p & lt ; 0.001 ) both showed stronger evidence of association with suspected or definite PLIKS .
	manualset3
213445	6	419567	7	NULL	NULL	0	NULL	CI 1.04	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although not a priori hypotheses , family history of depression ( adjusted OR = 1.28 , 95 % CI 1.04 , 1.57 ; p = 0.018 ) , and younger maternal age ( adjusted OR per 10-year age increase = 0.62 , 95 % CI 0.47 , 0.82 ; p & lt ; 0.001 ) both showed stronger evidence of association with suspected or definite PLIKS .
	manualset3
213446	7	419567	7	NULL	NULL	0	NULL	1.57	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Although not a priori hypotheses , family history of depression ( adjusted OR = 1.28 , 95 % CI 1.04 , 1.57 ; p = 0.018 ) , and younger maternal age ( adjusted OR per 10-year age increase = 0.62 , 95 % CI 0.47 , 0.82 ; p & lt ; 0.001 ) both showed stronger evidence of association with suspected or definite PLIKS .
	manualset3
213447	8	419567	7	NULL	NULL	0	NULL	p = 0.018	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Although not a priori hypotheses , family history of depression ( adjusted OR = 1.28 , 95 % CI 1.04 , 1.57 ; p = 0.018 ) , and younger maternal age ( adjusted OR per 10-year age increase = 0.62 , 95 % CI 0.47 , 0.82 ; p & lt ; 0.001 ) both showed stronger evidence of association with suspected or definite PLIKS .
	manualset3
213448	9	419567	7	NULL	NULL	0	NULL	younger maternal age	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although not a priori hypotheses , family history of depression ( adjusted OR = 1.28 , 95 % CI 1.04 , 1.57 ; p = 0.018 ) , and younger maternal age ( adjusted OR per 10-year age increase = 0.62 , 95 % CI 0.47 , 0.82 ; p & lt ; 0.001 ) both showed stronger evidence of association with suspected or definite PLIKS .
	manualset3
213449	10	419567	7	NULL	NULL	NULL	NULL	OR per 10-year age increase	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although not a priori hypotheses , family history of depression ( adjusted OR = 1.28 , 95 % CI 1.04 , 1.57 ; p = 0.018 ) , and younger maternal age ( adjusted OR per 10-year age increase = 0.62 , 95 % CI 0.47 , 0.82 ; p & lt ; 0.001 ) both showed stronger evidence of association with suspected or definite PLIKS .
	manualset3
213450	11	419567	7	NULL	NULL	0	NULL	0.62	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Although not a priori hypotheses , family history of depression ( adjusted OR = 1.28 , 95 % CI 1.04 , 1.57 ; p = 0.018 ) , and younger maternal age ( adjusted OR per 10-year age increase = 0.62 , 95 % CI 0.47 , 0.82 ; p & lt ; 0.001 ) both showed stronger evidence of association with suspected or definite PLIKS .
	manualset3
213451	12	419567	7	NULL	NULL	0	NULL	95 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although not a priori hypotheses , family history of depression ( adjusted OR = 1.28 , 95 % CI 1.04 , 1.57 ; p = 0.018 ) , and younger maternal age ( adjusted OR per 10-year age increase = 0.62 , 95 % CI 0.47 , 0.82 ; p & lt ; 0.001 ) both showed stronger evidence of association with suspected or definite PLIKS .
	manualset3
213452	13	419567	7	NULL	NULL	0	NULL	CI 0.47	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although not a priori hypotheses , family history of depression ( adjusted OR = 1.28 , 95 % CI 1.04 , 1.57 ; p = 0.018 ) , and younger maternal age ( adjusted OR per 10-year age increase = 0.62 , 95 % CI 0.47 , 0.82 ; p & lt ; 0.001 ) both showed stronger evidence of association with suspected or definite PLIKS .
	manualset3
213453	14	419567	7	NULL	NULL	0	NULL	0.82	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Although not a priori hypotheses , family history of depression ( adjusted OR = 1.28 , 95 % CI 1.04 , 1.57 ; p = 0.018 ) , and younger maternal age ( adjusted OR per 10-year age increase = 0.62 , 95 % CI 0.47 , 0.82 ; p & lt ; 0.001 ) both showed stronger evidence of association with suspected or definite PLIKS .
	manualset3
213454	15	419567	7	NULL	NULL	0	NULL	p & lt ; 0.001	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although not a priori hypotheses , family history of depression ( adjusted OR = 1.28 , 95 % CI 1.04 , 1.57 ; p = 0.018 ) , and younger maternal age ( adjusted OR per 10-year age increase = 0.62 , 95 % CI 0.47 , 0.82 ; p & lt ; 0.001 ) both showed stronger evidence of association with suspected or definite PLIKS .
	manualset3
213455	16	419567	7	NULL	NULL	0	NULL	stronger evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although not a priori hypotheses , family history of depression ( adjusted OR = 1.28 , 95 % CI 1.04 , 1.57 ; p = 0.018 ) , and younger maternal age ( adjusted OR per 10-year age increase = 0.62 , 95 % CI 0.47 , 0.82 ; p & lt ; 0.001 ) both showed stronger evidence of association with suspected or definite PLIKS .
	manualset3
213456	17	419567	7	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Although not a priori hypotheses , family history of depression ( adjusted OR = 1.28 , 95 % CI 1.04 , 1.57 ; p = 0.018 ) , and younger maternal age ( adjusted OR per 10-year age increase = 0.62 , 95 % CI 0.47 , 0.82 ; p & lt ; 0.001 ) both showed stronger evidence of association with suspected or definite PLIKS .
	manualset3
213457	18	419567	7	NULL	NULL	0	NULL	suspected or definite PLIKS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although not a priori hypotheses , family history of depression ( adjusted OR = 1.28 , 95 % CI 1.04 , 1.57 ; p = 0.018 ) , and younger maternal age ( adjusted OR per 10-year age increase = 0.62 , 95 % CI 0.47 , 0.82 ; p & lt ; 0.001 ) both showed stronger evidence of association with suspected or definite PLIKS .
	manualset3
213458	1	419568	7	NULL	NULL	NULL	NULL	 morphological similarities	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The morphological and habitat similarities of Philcoxia to those of some carnivorous plants , along with recent observations of nematodes over its subterranean leaves , prompted the suggestion that the genus is carnivorous .
	manualset3
213459	2	419568	7	NULL	NULL	NULL	NULL	habitat similarities	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The morphological and habitat similarities of Philcoxia to those of some carnivorous plants , along with recent observations of nematodes over its subterranean leaves , prompted the suggestion that the genus is carnivorous .
	manualset3
213460	3	419568	7	NULL	NULL	0	NULL	Philcoxia	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological and habitat similarities of Philcoxia to those of some carnivorous plants , along with recent observations of nematodes over its subterranean leaves , prompted the suggestion that the genus is carnivorous .
	manualset3
213461	4	419568	7	NULL	NULL	0	NULL	carnivorous plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological and habitat similarities of Philcoxia to those of some carnivorous plants , along with recent observations of nematodes over its subterranean leaves , prompted the suggestion that the genus is carnivorous .
	manualset3
213462	5	419568	7	NULL	NULL	0	NULL	recent observations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological and habitat similarities of Philcoxia to those of some carnivorous plants , along with recent observations of nematodes over its subterranean leaves , prompted the suggestion that the genus is carnivorous .
	manualset3
213463	6	419568	7	NULL	NULL	0	NULL	nematodes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological and habitat similarities of Philcoxia to those of some carnivorous plants , along with recent observations of nematodes over its subterranean leaves , prompted the suggestion that the genus is carnivorous .
	manualset3
213464	7	419568	7	NULL	NULL	0	NULL	subterranean leaves	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological and habitat similarities of Philcoxia to those of some carnivorous plants , along with recent observations of nematodes over its subterranean leaves , prompted the suggestion that the genus is carnivorous .
	manualset3
213465	8	419568	7	NULL	NULL	0	NULL	genus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological and habitat similarities of Philcoxia to those of some carnivorous plants , along with recent observations of nematodes over its subterranean leaves , prompted the suggestion that the genus is carnivorous .
	manualset3
213466	9	419568	7	NULL	NULL	0	NULL	carnivorous 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological and habitat similarities of Philcoxia to those of some carnivorous plants , along with recent observations of nematodes over its subterranean leaves , prompted the suggestion that the genus is carnivorous .
	manualset3
214850	10	419568	7	NULL	NULL	0	NULL	suggestion	process												NULL		0	NULL	NULL	NULL	NULL	NULL	The morphological and habitat similarities of Philcoxia to those of some carnivorous plants , along with recent observations of nematodes over its subterranean leaves , prompted the suggestion that the genus is carnivorous .
	manualset3
213467	1	419569	7	NULL	NULL	0	NULL	 human T-cell leukemia virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The human T-cell leukemia virus Tax protein influences transcription through interactions with cellular proteins in the nucleus as well as the cytoplasm .
	manualset3
213468	2	419569	7	NULL	NULL	0	NULL	Tax protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The human T-cell leukemia virus Tax protein influences transcription through interactions with cellular proteins in the nucleus as well as the cytoplasm .
	manualset3
213469	3	419569	7	NULL	NULL	0	NULL	transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The human T-cell leukemia virus Tax protein influences transcription through interactions with cellular proteins in the nucleus as well as the cytoplasm .
	manualset3
213470	4	419569	7	NULL	NULL	0	NULL	interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The human T-cell leukemia virus Tax protein influences transcription through interactions with cellular proteins in the nucleus as well as the cytoplasm .
	manualset3
213471	5	419569	7	NULL	NULL	0	NULL	cellular proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The human T-cell leukemia virus Tax protein influences transcription through interactions with cellular proteins in the nucleus as well as the cytoplasm .
	manualset3
213472	6	419569	7	NULL	NULL	0	NULL	nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The human T-cell leukemia virus Tax protein influences transcription through interactions with cellular proteins in the nucleus as well as the cytoplasm .
	manualset3
213473	7	419569	7	NULL	NULL	0	NULL	cytoplasm	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The human T-cell leukemia virus Tax protein influences transcription through interactions with cellular proteins in the nucleus as well as the cytoplasm .
	manualset3
213474	1	419570	7	NULL	NULL	0	NULL	 tolazamide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Value of tolazamide '' ` Tolanase ' ) as an oral hypoglycaemic agent .
	manualset3
213475	2	419570	7	NULL	NULL	0	NULL	Tolanase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Value of tolazamide '' ` Tolanase ' ) as an oral hypoglycaemic agent .
	manualset3
213476	3	419570	7	NULL	NULL	0	NULL	oral hypoglycaemic agent	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Value of tolazamide '' ` Tolanase ' ) as an oral hypoglycaemic agent .
	manualset3
213477	1	419571	7	NULL	NULL	0	NULL	role 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of ultraviolet light in the induction of cellular DNA damage by a spark-gap lithotripter in vitro .
	manualset3
213478	2	419571	7	NULL	NULL	0	NULL	ultraviolet light	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of ultraviolet light in the induction of cellular DNA damage by a spark-gap lithotripter in vitro .
	manualset3
213479	3	419571	7	NULL	NULL	0	NULL	induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of ultraviolet light in the induction of cellular DNA damage by a spark-gap lithotripter in vitro .
	manualset3
213480	4	419571	7	NULL	NULL	0	NULL	cellular DNA damage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of ultraviolet light in the induction of cellular DNA damage by a spark-gap lithotripter in vitro .
	manualset3
213481	5	419571	7	NULL	NULL	0	NULL	spark-gap lithotripter	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of ultraviolet light in the induction of cellular DNA damage by a spark-gap lithotripter in vitro .
	manualset3
213482	1	419572	7	NULL	NULL	NULL	NULL	increased peroxidation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Significantly increased peroxidation was observed in intact erythrocytes , isolated lipids from intact erythrocytes or their ghosts compared with normal controls .
	manualset3
213483	2	419572	7	NULL	NULL	0	NULL	intact erythrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Significantly increased peroxidation was observed in intact erythrocytes , isolated lipids from intact erythrocytes or their ghosts compared with normal controls .
	manualset3
213484	3	419572	7	NULL	NULL	0	NULL	 isolated lipids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Significantly increased peroxidation was observed in intact erythrocytes , isolated lipids from intact erythrocytes or their ghosts compared with normal controls .
	manualset3
213485	4	419572	7	NULL	NULL	0	NULL	intact erythrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Significantly increased peroxidation was observed in intact erythrocytes , isolated lipids from intact erythrocytes or their ghosts compared with normal controls .
	manualset3
213486	5	419572	7	NULL	NULL	0	NULL	ghosts 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Significantly increased peroxidation was observed in intact erythrocytes , isolated lipids from intact erythrocytes or their ghosts compared with normal controls .
	manualset3
213487	6	419572	7	NULL	NULL	0	NULL	normal controls	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Significantly increased peroxidation was observed in intact erythrocytes , isolated lipids from intact erythrocytes or their ghosts compared with normal controls .
	manualset3
213488	1	419573	7	NULL	NULL	NULL	NULL	Anatomical characterization	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Anatomical characterization of a novel reticulospinal vasodepressor area in the rat medulla oblongata .
	manualset3
213489	2	419573	7	NULL	NULL	0	NULL	novel reticulospinal vasodepressor area	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomical characterization of a novel reticulospinal vasodepressor area in the rat medulla oblongata .
	manualset3
213490	3	419573	7	NULL	NULL	0	NULL	rat medulla oblongata 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomical characterization of a novel reticulospinal vasodepressor area in the rat medulla oblongata .
	manualset3
213491	1	419574	7	NULL	NULL	0	NULL	 Importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Importance of studying deficiencies of IgG subclasses ( IgG2 and IgG4 ) in immuno-allergologic practice ) .
	manualset3
213492	2	419574	7	NULL	NULL	0	NULL	deficiencies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Importance of studying deficiencies of IgG subclasses ( IgG2 and IgG4 ) in immuno-allergologic practice ) .
	manualset3
213493	3	419574	7	NULL	NULL	0	NULL	IgG subclasses 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Importance of studying deficiencies of IgG subclasses ( IgG2 and IgG4 ) in immuno-allergologic practice ) .
	manualset3
213494	4	419574	7	NULL	NULL	0	NULL	IgG2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Importance of studying deficiencies of IgG subclasses ( IgG2 and IgG4 ) in immuno-allergologic practice ) .
	manualset3
213495	5	419574	7	NULL	NULL	0	NULL	IgG4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Importance of studying deficiencies of IgG subclasses ( IgG2 and IgG4 ) in immuno-allergologic practice ) .
	manualset3
213496	6	419574	7	NULL	NULL	0	NULL	immuno-allergologic practice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Importance of studying deficiencies of IgG subclasses ( IgG2 and IgG4 ) in immuno-allergologic practice ) .
	manualset3
213497	1	419575	7	NULL	NULL	0	NULL	Limitations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Limitations to physician liability are discussed for transferred data .
	manualset3
213498	2	419575	7	NULL	NULL	0	NULL	physician liability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Limitations to physician liability are discussed for transferred data .
	manualset3
213499	3	419575	7	NULL	NULL	0	NULL	transferred data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Limitations to physician liability are discussed for transferred data .
	manualset3
213500	1	419576	7	NULL	NULL	0	NULL	Outbreak	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Outbreak of hepatitis A in a day-care institution ) .
	manualset3
213501	2	419576	7	NULL	NULL	0	NULL	hepatitis A	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Outbreak of hepatitis A in a day-care institution ) .
	manualset3
213502	3	419576	7	NULL	NULL	0	NULL	day-care institution	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( Outbreak of hepatitis A in a day-care institution ) .
	manualset3
213503	1	419577	7	NULL	NULL	0	NULL	Primiparae	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Primiparae in their early 30s may be one of the first selection criteria for CB donors to obtain higher yield of TNC .
	manualset3
213504	2	419577	7	NULL	NULL	0	NULL	early 30s	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Primiparae in their early 30s may be one of the first selection criteria for CB donors to obtain higher yield of TNC .
	manualset3
213505	3	419577	7	NULL	NULL	0	NULL	first selection criteria	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Primiparae in their early 30s may be one of the first selection criteria for CB donors to obtain higher yield of TNC .
	manualset3
213506	4	419577	7	NULL	NULL	0	NULL	CB donors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Primiparae in their early 30s may be one of the first selection criteria for CB donors to obtain higher yield of TNC .
	manualset3
213507	5	419577	7	NULL	NULL	0	NULL	higher yield	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Primiparae in their early 30s may be one of the first selection criteria for CB donors to obtain higher yield of TNC .
	manualset3
213508	6	419577	7	NULL	NULL	0	NULL	TNC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Primiparae in their early 30s may be one of the first selection criteria for CB donors to obtain higher yield of TNC .
	manualset3
213509	1	419578	7	NULL	NULL	0	NULL	Difficult employees 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Difficult employees : a management challenge .
	manualset3
213510	2	419578	7	NULL	NULL	0	NULL	management challenge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Difficult employees : a management challenge .
	manualset3
213511	1	419579	7	NULL	NULL	0	NULL	 field	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	As the field of neuro-oncology expands , the neuroscience nurse needs to develop an understanding of clinical trials and their operation .
	manualset3
213512	2	419579	7	NULL	NULL	0	NULL	 neuro-oncology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	As the field of neuro-oncology expands , the neuroscience nurse needs to develop an understanding of clinical trials and their operation .
	manualset3
213513	3	419579	7	NULL	NULL	0	NULL	neuroscience nurse	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	As the field of neuro-oncology expands , the neuroscience nurse needs to develop an understanding of clinical trials and their operation .
	manualset3
213514	4	419579	7	NULL	NULL	0	NULL	understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As the field of neuro-oncology expands , the neuroscience nurse needs to develop an understanding of clinical trials and their operation .
	manualset3
213515	5	419579	7	NULL	NULL	NULL	NULL	clinical trials 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As the field of neuro-oncology expands , the neuroscience nurse needs to develop an understanding of clinical trials and their operation .
	manualset3
213516	6	419579	7	NULL	NULL	0	NULL	operation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As the field of neuro-oncology expands , the neuroscience nurse needs to develop an understanding of clinical trials and their operation .
	manualset3
213517	1	419580	7	NULL	NULL	0	NULL	Effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of dietary olive oil on plasma high density lipoproteins ) .
	manualset3
213518	2	419580	7	NULL	NULL	0	NULL	dietary olive oil 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of dietary olive oil on plasma high density lipoproteins ) .
	manualset3
213519	3	419580	7	NULL	NULL	NULL	NULL	plasma high density lipoproteins	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Effect of dietary olive oil on plasma high density lipoproteins ) .
	manualset3
213520	1	419581	7	NULL	NULL	0	NULL	Lin-2	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Lin-2 encodes a MAGUK and lin-7 encodes a small protein with one PDZ domain .
	manualset3
213521	2	419581	7	NULL	NULL	0	NULL	MAGUK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lin-2 encodes a MAGUK and lin-7 encodes a small protein with one PDZ domain .
	manualset3
213522	3	419581	7	NULL	NULL	0	NULL	lin-7	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Lin-2 encodes a MAGUK and lin-7 encodes a small protein with one PDZ domain .
	manualset3
213523	4	419581	7	NULL	NULL	0	NULL	small protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lin-2 encodes a MAGUK and lin-7 encodes a small protein with one PDZ domain .
	manualset3
213524	5	419581	7	NULL	NULL	0	NULL	one PDZ domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lin-2 encodes a MAGUK and lin-7 encodes a small protein with one PDZ domain .
	manualset3
213525	1	419582	7	NULL	NULL	0	NULL	Serum CK-MB levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum CK-MB levels are most helpful clinically when the total creatine kinase is nonspecifically elevated , as with intramuscular injections , cardiac catheterization , stroke , noncardiac surgery and electric cardioversion .
	manualset3
213526	2	419582	7	NULL	NULL	0	NULL	 total creatine kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum CK-MB levels are most helpful clinically when the total creatine kinase is nonspecifically elevated , as with intramuscular injections , cardiac catheterization , stroke , noncardiac surgery and electric cardioversion .
	manualset3
213527	3	419582	7	NULL	NULL	0	NULL	 intramuscular injections	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum CK-MB levels are most helpful clinically when the total creatine kinase is nonspecifically elevated , as with intramuscular injections , cardiac catheterization , stroke , noncardiac surgery and electric cardioversion .
	manualset3
213528	4	419582	7	NULL	NULL	0	NULL	cardiac catheterization 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum CK-MB levels are most helpful clinically when the total creatine kinase is nonspecifically elevated , as with intramuscular injections , cardiac catheterization , stroke , noncardiac surgery and electric cardioversion .
	manualset3
213529	5	419582	7	NULL	NULL	0	NULL	stroke	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum CK-MB levels are most helpful clinically when the total creatine kinase is nonspecifically elevated , as with intramuscular injections , cardiac catheterization , stroke , noncardiac surgery and electric cardioversion .
	manualset3
213530	6	419582	7	NULL	NULL	0	NULL	noncardiac surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum CK-MB levels are most helpful clinically when the total creatine kinase is nonspecifically elevated , as with intramuscular injections , cardiac catheterization , stroke , noncardiac surgery and electric cardioversion .
	manualset3
213531	7	419582	7	NULL	NULL	0	NULL	electric cardioversion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum CK-MB levels are most helpful clinically when the total creatine kinase is nonspecifically elevated , as with intramuscular injections , cardiac catheterization , stroke , noncardiac surgery and electric cardioversion .
	manualset3
213532	1	419583	7	NULL	NULL	0	NULL	Development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Development of states of physiologic stress in sailors during cruises in low latitudes ) .
	manualset3
213533	2	419583	7	NULL	NULL	0	NULL	states	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Development of states of physiologic stress in sailors during cruises in low latitudes ) .
	manualset3
213534	3	419583	7	NULL	NULL	0	NULL	physiologic stress 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Development of states of physiologic stress in sailors during cruises in low latitudes ) .
	manualset3
213535	4	419583	7	NULL	NULL	0	NULL	sailors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Development of states of physiologic stress in sailors during cruises in low latitudes ) .
	manualset3
213536	5	419583	7	NULL	NULL	0	NULL	cruises	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Development of states of physiologic stress in sailors during cruises in low latitudes ) .
	manualset3
213537	6	419583	7	NULL	NULL	0	NULL	low latitudes	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Development of states of physiologic stress in sailors during cruises in low latitudes ) .
	manualset3
213538	1	419584	7	NULL	NULL	0	NULL	Longevity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Longevity was linked to LRS via a chain of statistically significant relationships : The longer the life span , the longer the reproductive life ; the longer the reproductive life , the more offspring produced ; the more offspring produced , the higher the LRS .
	manualset3
213539	2	419584	7	NULL	NULL	0	NULL	LRS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Longevity was linked to LRS via a chain of statistically significant relationships : The longer the life span , the longer the reproductive life ; the longer the reproductive life , the more offspring produced ; the more offspring produced , the higher the LRS .
	manualset3
213540	3	419584	7	NULL	NULL	0	NULL	chain	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Longevity was linked to LRS via a chain of statistically significant relationships : The longer the life span , the longer the reproductive life ; the longer the reproductive life , the more offspring produced ; the more offspring produced , the higher the LRS .
	manualset3
213541	4	419584	7	NULL	NULL	0	NULL	statistically significant relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Longevity was linked to LRS via a chain of statistically significant relationships : The longer the life span , the longer the reproductive life ; the longer the reproductive life , the more offspring produced ; the more offspring produced , the higher the LRS .
	manualset3
213542	5	419584	7	NULL	NULL	0	NULL	 life span	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Longevity was linked to LRS via a chain of statistically significant relationships : The longer the life span , the longer the reproductive life ; the longer the reproductive life , the more offspring produced ; the more offspring produced , the higher the LRS .
	manualset3
213543	6	419584	7	NULL	NULL	0	NULL	reproductive life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Longevity was linked to LRS via a chain of statistically significant relationships : The longer the life span , the longer the reproductive life ; the longer the reproductive life , the more offspring produced ; the more offspring produced , the higher the LRS .
	manualset3
213544	7	419584	7	NULL	NULL	0	NULL	reproductive life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Longevity was linked to LRS via a chain of statistically significant relationships : The longer the life span , the longer the reproductive life ; the longer the reproductive life , the more offspring produced ; the more offspring produced , the higher the LRS .
	manualset3
213545	8	419584	7	NULL	NULL	0	NULL	offspring	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Longevity was linked to LRS via a chain of statistically significant relationships : The longer the life span , the longer the reproductive life ; the longer the reproductive life , the more offspring produced ; the more offspring produced , the higher the LRS .
	manualset3
213546	9	419584	7	NULL	NULL	0	NULL	 offspring	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Longevity was linked to LRS via a chain of statistically significant relationships : The longer the life span , the longer the reproductive life ; the longer the reproductive life , the more offspring produced ; the more offspring produced , the higher the LRS .
	manualset3
213547	10	419584	7	NULL	NULL	0	NULL	 LRS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Longevity was linked to LRS via a chain of statistically significant relationships : The longer the life span , the longer the reproductive life ; the longer the reproductive life , the more offspring produced ; the more offspring produced , the higher the LRS .
	manualset3
213548	1	419585	7	NULL	NULL	0	NULL	Availability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Availability of recombinant growth hormone ( GH ) and development of long-acting formulations of this material will undoubtedly lead to widespread use of GH in animal industry and in medicine .
	manualset3
213549	2	419585	7	NULL	NULL	0	NULL	recombinant growth hormone ( GH )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Availability of recombinant growth hormone ( GH ) and development of long-acting formulations of this material will undoubtedly lead to widespread use of GH in animal industry and in medicine .
	manualset3
213550	3	419585	7	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Availability of recombinant growth hormone ( GH ) and development of long-acting formulations of this material will undoubtedly lead to widespread use of GH in animal industry and in medicine .
	manualset3
213551	4	419585	7	NULL	NULL	0	NULL	long-acting formulations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Availability of recombinant growth hormone ( GH ) and development of long-acting formulations of this material will undoubtedly lead to widespread use of GH in animal industry and in medicine .
	manualset3
213552	5	419585	7	NULL	NULL	0	NULL	material	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Availability of recombinant growth hormone ( GH ) and development of long-acting formulations of this material will undoubtedly lead to widespread use of GH in animal industry and in medicine .
	manualset3
213553	6	419585	7	NULL	NULL	0	NULL	use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Availability of recombinant growth hormone ( GH ) and development of long-acting formulations of this material will undoubtedly lead to widespread use of GH in animal industry and in medicine .
	manualset3
213554	7	419585	7	NULL	NULL	0	NULL	GH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Availability of recombinant growth hormone ( GH ) and development of long-acting formulations of this material will undoubtedly lead to widespread use of GH in animal industry and in medicine .
	manualset3
213555	8	419585	7	NULL	NULL	0	NULL	animal industry	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Availability of recombinant growth hormone ( GH ) and development of long-acting formulations of this material will undoubtedly lead to widespread use of GH in animal industry and in medicine .
	manualset3
213556	9	419585	7	NULL	NULL	0	NULL	medicine	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Availability of recombinant growth hormone ( GH ) and development of long-acting formulations of this material will undoubtedly lead to widespread use of GH in animal industry and in medicine .
	manualset3
213557	1	419586	7	NULL	NULL	0	NULL	mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mutation was C to A transversion substituting lysine ( AAG ) for normal glutamine ( CAG ) codon .
	manualset3
213558	2	419586	7	NULL	NULL	0	NULL	C to A transversion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mutation was C to A transversion substituting lysine ( AAG ) for normal glutamine ( CAG ) codon .
	manualset3
213559	3	419586	7	NULL	NULL	NULL	NULL	lysine ( AAG ) codon	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The mutation was C to A transversion substituting lysine ( AAG ) for normal glutamine ( CAG ) codon .
	manualset3
213560	4	419586	7	NULL	NULL	NULL	NULL	glutamine ( CAG ) codon 	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The mutation was C to A transversion substituting lysine ( AAG ) for normal glutamine ( CAG ) codon .
	manualset3
213561	1	419587	7	NULL	NULL	0	NULL	Polymerase chain reaction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Polymerase chain reaction in the demonstration of Borrelia burgdorferi DNA ) .
	manualset3
213562	2	419587	7	NULL	NULL	0	NULL	demonstration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Polymerase chain reaction in the demonstration of Borrelia burgdorferi DNA ) .
	manualset3
213563	3	419587	7	NULL	NULL	0	NULL	Borrelia burgdorferi DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	( Polymerase chain reaction in the demonstration of Borrelia burgdorferi DNA ) .
	manualset3
213565	1	419588	7	NULL	NULL	0	NULL	order	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The order of binding to poly ( A ) was ; 7 , 12-dimethylbenza ( a ) anthracene greater than benzo ( a ) pyrene greater than dibenz ( a , h ) anthracene greater than dibenz ( a , c ) anthracene .
	manualset3
213566	2	419588	7	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The order of binding to poly ( A ) was ; 7 , 12-dimethylbenza ( a ) anthracene greater than benzo ( a ) pyrene greater than dibenz ( a , h ) anthracene greater than dibenz ( a , c ) anthracene .
	manualset3
213567	3	419588	7	NULL	NULL	0	NULL	poly ( A )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The order of binding to poly ( A ) was ; 7 , 12-dimethylbenza ( a ) anthracene greater than benzo ( a ) pyrene greater than dibenz ( a , h ) anthracene greater than dibenz ( a , c ) anthracene .
	manualset3
213568	4	419588	7	NULL	NULL	0	NULL	7 , 12-dimethylbenza ( a ) anthracene 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The order of binding to poly ( A ) was ; 7 , 12-dimethylbenza ( a ) anthracene greater than benzo ( a ) pyrene greater than dibenz ( a , h ) anthracene greater than dibenz ( a , c ) anthracene .
	manualset3
213569	5	419588	7	NULL	NULL	0	NULL	benzo ( a ) pyrene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The order of binding to poly ( A ) was ; 7 , 12-dimethylbenza ( a ) anthracene greater than benzo ( a ) pyrene greater than dibenz ( a , h ) anthracene greater than dibenz ( a , c ) anthracene .
	manualset3
213570	6	419588	7	NULL	NULL	0	NULL	dibenz ( a , h ) anthracene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The order of binding to poly ( A ) was ; 7 , 12-dimethylbenza ( a ) anthracene greater than benzo ( a ) pyrene greater than dibenz ( a , h ) anthracene greater than dibenz ( a , c ) anthracene .
	manualset3
213571	7	419588	7	NULL	NULL	0	NULL	 dibenz ( a , c ) anthracene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The order of binding to poly ( A ) was ; 7 , 12-dimethylbenza ( a ) anthracene greater than benzo ( a ) pyrene greater than dibenz ( a , h ) anthracene greater than dibenz ( a , c ) anthracene .
	manualset3
213572	1	419589	7	NULL	NULL	0	NULL	Histological changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological changes which appear as a result of reperfusion injury of cold-preserved rat liver were studied at intervals of 0 hr , 3 hr , 24 hr and 48 hr of cold storage .
	manualset3
213573	2	419589	7	NULL	NULL	0	NULL	result	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological changes which appear as a result of reperfusion injury of cold-preserved rat liver were studied at intervals of 0 hr , 3 hr , 24 hr and 48 hr of cold storage .
	manualset3
213574	3	419589	7	NULL	NULL	0	NULL	reperfusion injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological changes which appear as a result of reperfusion injury of cold-preserved rat liver were studied at intervals of 0 hr , 3 hr , 24 hr and 48 hr of cold storage .
	manualset3
213575	4	419589	7	NULL	NULL	0	NULL	cold-preserved rat liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological changes which appear as a result of reperfusion injury of cold-preserved rat liver were studied at intervals of 0 hr , 3 hr , 24 hr and 48 hr of cold storage .
	manualset3
213576	5	419589	7	NULL	NULL	0	NULL	intervals	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological changes which appear as a result of reperfusion injury of cold-preserved rat liver were studied at intervals of 0 hr , 3 hr , 24 hr and 48 hr of cold storage .
	manualset3
213577	6	419589	7	NULL	NULL	0	NULL	 0 hr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological changes which appear as a result of reperfusion injury of cold-preserved rat liver were studied at intervals of 0 hr , 3 hr , 24 hr and 48 hr of cold storage .
	manualset3
213578	7	419589	7	NULL	NULL	0	NULL	3 hr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological changes which appear as a result of reperfusion injury of cold-preserved rat liver were studied at intervals of 0 hr , 3 hr , 24 hr and 48 hr of cold storage .
	manualset3
213579	8	419589	7	NULL	NULL	0	NULL	24 hr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological changes which appear as a result of reperfusion injury of cold-preserved rat liver were studied at intervals of 0 hr , 3 hr , 24 hr and 48 hr of cold storage .
	manualset3
213580	9	419589	7	NULL	NULL	0	NULL	48 hr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological changes which appear as a result of reperfusion injury of cold-preserved rat liver were studied at intervals of 0 hr , 3 hr , 24 hr and 48 hr of cold storage .
	manualset3
213581	10	419589	7	NULL	NULL	0	NULL	cold storage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Histological changes which appear as a result of reperfusion injury of cold-preserved rat liver were studied at intervals of 0 hr , 3 hr , 24 hr and 48 hr of cold storage .
	manualset3
213582	1	419590	7	NULL	NULL	0	NULL	DU 145 cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Since DU 145 cells have deficient gap junctions , intercellular bridges may have a prominent role in the transfer of chemical signals between these cells .
	manualset3
213583	2	419590	7	NULL	NULL	0	NULL	gap junctions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Since DU 145 cells have deficient gap junctions , intercellular bridges may have a prominent role in the transfer of chemical signals between these cells .
	manualset3
213584	3	419590	7	NULL	NULL	0	NULL	intercellular bridges 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Since DU 145 cells have deficient gap junctions , intercellular bridges may have a prominent role in the transfer of chemical signals between these cells .
	manualset3
213585	4	419590	7	NULL	NULL	0	NULL	prominent role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since DU 145 cells have deficient gap junctions , intercellular bridges may have a prominent role in the transfer of chemical signals between these cells .
	manualset3
213586	5	419590	7	NULL	NULL	0	NULL	transfer	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since DU 145 cells have deficient gap junctions , intercellular bridges may have a prominent role in the transfer of chemical signals between these cells .
	manualset3
213587	6	419590	7	NULL	NULL	0	NULL	chemical signals	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since DU 145 cells have deficient gap junctions , intercellular bridges may have a prominent role in the transfer of chemical signals between these cells .
	manualset3
213588	7	419590	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Since DU 145 cells have deficient gap junctions , intercellular bridges may have a prominent role in the transfer of chemical signals between these cells .
	manualset3
213589	1	419591	7	NULL	NULL	0	NULL	anodic peak currents	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The anodic peak currents increased linearly with the concentration of tryptophan in the range of 2.0 x10 ( -7 ) to 1.0 x10 ( -4 ) M with a detection limit of 2.0 x10 ( -8 ) M ( at a S/N = 3 ) .
	manualset3
213590	2	419591	7	NULL	NULL	0	NULL	 concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The anodic peak currents increased linearly with the concentration of tryptophan in the range of 2.0 x10 ( -7 ) to 1.0 x10 ( -4 ) M with a detection limit of 2.0 x10 ( -8 ) M ( at a S/N = 3 ) .
	manualset3
213591	3	419591	7	NULL	NULL	0	NULL	tryptophan	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The anodic peak currents increased linearly with the concentration of tryptophan in the range of 2.0 x10 ( -7 ) to 1.0 x10 ( -4 ) M with a detection limit of 2.0 x10 ( -8 ) M ( at a S/N = 3 ) .
	manualset3
213592	4	419591	7	NULL	NULL	0	NULL	range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The anodic peak currents increased linearly with the concentration of tryptophan in the range of 2.0 x10 ( -7 ) to 1.0 x10 ( -4 ) M with a detection limit of 2.0 x10 ( -8 ) M ( at a S/N = 3 ) .
	manualset3
213593	5	419591	7	NULL	NULL	0	NULL	2.0 x10 ( -7 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The anodic peak currents increased linearly with the concentration of tryptophan in the range of 2.0 x10 ( -7 ) to 1.0 x10 ( -4 ) M with a detection limit of 2.0 x10 ( -8 ) M ( at a S/N = 3 ) .
	manualset3
213594	6	419591	7	NULL	NULL	0	NULL	 1.0 x10 ( -4 ) M 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The anodic peak currents increased linearly with the concentration of tryptophan in the range of 2.0 x10 ( -7 ) to 1.0 x10 ( -4 ) M with a detection limit of 2.0 x10 ( -8 ) M ( at a S/N = 3 ) .
	manualset3
213595	7	419591	7	NULL	NULL	0	NULL	detection limit	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The anodic peak currents increased linearly with the concentration of tryptophan in the range of 2.0 x10 ( -7 ) to 1.0 x10 ( -4 ) M with a detection limit of 2.0 x10 ( -8 ) M ( at a S/N = 3 ) .
	manualset3
213596	8	419591	7	NULL	NULL	0	NULL	2.0 x10 ( -8 ) M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The anodic peak currents increased linearly with the concentration of tryptophan in the range of 2.0 x10 ( -7 ) to 1.0 x10 ( -4 ) M with a detection limit of 2.0 x10 ( -8 ) M ( at a S/N = 3 ) .
	manualset3
213597	9	419591	7	NULL	NULL	0	NULL	 S/N = 3	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The anodic peak currents increased linearly with the concentration of tryptophan in the range of 2.0 x10 ( -7 ) to 1.0 x10 ( -4 ) M with a detection limit of 2.0 x10 ( -8 ) M ( at a S/N = 3 ) .
	manualset3
213598	1	419592	7	NULL	NULL	0	NULL	HPV insertion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HPV insertion into the genome can cause permanent changes in cellular DNA that disturb the regulation of cell proliferation .
	manualset3
213599	2	419592	7	NULL	NULL	0	NULL	 genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	HPV insertion into the genome can cause permanent changes in cellular DNA that disturb the regulation of cell proliferation .
	manualset3
213600	3	419592	7	NULL	NULL	0	NULL	permanent changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HPV insertion into the genome can cause permanent changes in cellular DNA that disturb the regulation of cell proliferation .
	manualset3
213601	4	419592	7	NULL	NULL	0	NULL	cellular DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	HPV insertion into the genome can cause permanent changes in cellular DNA that disturb the regulation of cell proliferation .
	manualset3
213602	5	419592	7	NULL	NULL	0	NULL	regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HPV insertion into the genome can cause permanent changes in cellular DNA that disturb the regulation of cell proliferation .
	manualset3
213603	6	419592	7	NULL	NULL	0	NULL	cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HPV insertion into the genome can cause permanent changes in cellular DNA that disturb the regulation of cell proliferation .
	manualset3
213604	1	419593	7	NULL	NULL	0	NULL	Small-angle x-ray scattering 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Small-angle x-ray scattering of human serum high-density lipoproteins .
	manualset3
213605	2	419593	7	NULL	NULL	0	NULL	human serum high-density lipoproteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Small-angle x-ray scattering of human serum high-density lipoproteins .
	manualset3
213606	1	419594	7	NULL	NULL	NULL	NULL	Two crown ether chemosensors	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Two crown ether chemosensors featuring a boron azadipyrrin chromophore have been synthesized ; both have absorption maxima at 650 nm , where all the shellfish extracts are transparent .
	manualset3
213607	2	419594	7	NULL	NULL	0	NULL	boron azadipyrrin chromophore	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two crown ether chemosensors featuring a boron azadipyrrin chromophore have been synthesized ; both have absorption maxima at 650 nm , where all the shellfish extracts are transparent .
	manualset3
213608	3	419594	7	NULL	NULL	0	NULL	absorption maxima	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two crown ether chemosensors featuring a boron azadipyrrin chromophore have been synthesized ; both have absorption maxima at 650 nm , where all the shellfish extracts are transparent .
	manualset3
213609	4	419594	7	NULL	NULL	0	NULL	 650 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Two crown ether chemosensors featuring a boron azadipyrrin chromophore have been synthesized ; both have absorption maxima at 650 nm , where all the shellfish extracts are transparent .
	manualset3
213610	5	419594	7	NULL	NULL	0	NULL	 shellfish extracts 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two crown ether chemosensors featuring a boron azadipyrrin chromophore have been synthesized ; both have absorption maxima at 650 nm , where all the shellfish extracts are transparent .
	manualset3
213611	1	419595	7	NULL	NULL	0	NULL	Postoperative angiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative angiography and computerised tomography were performed in 10 patients 8 to 57 months after surgical repair ( nine composite , one distal graft ) of aneurysms of the thoracic aorta ( six dissecting , four true aneurysms ) .
	manualset3
213612	2	419595	7	NULL	NULL	0	NULL	 computerised tomography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative angiography and computerised tomography were performed in 10 patients 8 to 57 months after surgical repair ( nine composite , one distal graft ) of aneurysms of the thoracic aorta ( six dissecting , four true aneurysms ) .
	manualset3
213613	3	419595	7	NULL	NULL	0	NULL	 10 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative angiography and computerised tomography were performed in 10 patients 8 to 57 months after surgical repair ( nine composite , one distal graft ) of aneurysms of the thoracic aorta ( six dissecting , four true aneurysms ) .
	manualset3
213614	4	419595	7	NULL	NULL	0	NULL	8 to 57 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative angiography and computerised tomography were performed in 10 patients 8 to 57 months after surgical repair ( nine composite , one distal graft ) of aneurysms of the thoracic aorta ( six dissecting , four true aneurysms ) .
	manualset3
213615	5	419595	7	NULL	NULL	0	NULL	surgical repair	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative angiography and computerised tomography were performed in 10 patients 8 to 57 months after surgical repair ( nine composite , one distal graft ) of aneurysms of the thoracic aorta ( six dissecting , four true aneurysms ) .
	manualset3
213616	6	419595	7	NULL	NULL	0	NULL	 nine composite	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative angiography and computerised tomography were performed in 10 patients 8 to 57 months after surgical repair ( nine composite , one distal graft ) of aneurysms of the thoracic aorta ( six dissecting , four true aneurysms ) .
	manualset3
213617	7	419595	7	NULL	NULL	0	NULL	one distal graft	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative angiography and computerised tomography were performed in 10 patients 8 to 57 months after surgical repair ( nine composite , one distal graft ) of aneurysms of the thoracic aorta ( six dissecting , four true aneurysms ) .
	manualset3
213618	8	419595	7	NULL	NULL	0	NULL	aneurysms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative angiography and computerised tomography were performed in 10 patients 8 to 57 months after surgical repair ( nine composite , one distal graft ) of aneurysms of the thoracic aorta ( six dissecting , four true aneurysms ) .
	manualset3
213619	9	419595	7	NULL	NULL	0	NULL	thoracic aorta 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative angiography and computerised tomography were performed in 10 patients 8 to 57 months after surgical repair ( nine composite , one distal graft ) of aneurysms of the thoracic aorta ( six dissecting , four true aneurysms ) .
	manualset3
213620	10	419595	7	NULL	NULL	0	NULL	six dissecting aneurysms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative angiography and computerised tomography were performed in 10 patients 8 to 57 months after surgical repair ( nine composite , one distal graft ) of aneurysms of the thoracic aorta ( six dissecting , four true aneurysms ) .
	manualset3
213621	11	419595	7	NULL	NULL	0	NULL	four true aneurysms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Postoperative angiography and computerised tomography were performed in 10 patients 8 to 57 months after surgical repair ( nine composite , one distal graft ) of aneurysms of the thoracic aorta ( six dissecting , four true aneurysms ) .
	manualset3
213622	1	419596	7	NULL	NULL	0	NULL	Fever	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Fever , diarrhea , and enlarging abdominal mass .
	manualset3
213623	2	419596	7	NULL	NULL	0	NULL	diarrhea	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Fever , diarrhea , and enlarging abdominal mass .
	manualset3
213624	3	419596	7	NULL	NULL	0	NULL	enlarging abdominal mass	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Fever , diarrhea , and enlarging abdominal mass .
	manualset3
213625	1	419597	7	NULL	NULL	0	NULL	Thyroid peroxidase antibodies	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thyroid peroxidase antibodies were absent in both patients .
	manualset3
213626	2	419597	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thyroid peroxidase antibodies were absent in both patients .
	manualset3
213627	1	419598	7	NULL	NULL	0	NULL	HIV testing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	HIV testing of infants : privacy and public health .
	manualset3
213628	2	419598	7	NULL	NULL	0	NULL	infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	HIV testing of infants : privacy and public health .
	manualset3
213629	3	419598	7	NULL	NULL	0	NULL	privacy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	HIV testing of infants : privacy and public health .
	manualset3
213630	4	419598	7	NULL	NULL	0	NULL	public health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	HIV testing of infants : privacy and public health .
	manualset3
213631	1	419599	7	NULL	NULL	0	NULL	mass ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In regard to the mass ratio , although the mass ratio of calcium to phosphorus was almost constant , the mass ratios of magnesium to calcium and phosphorus were different at early and advanced stages of the accumulation of calcium and phosphorus .
	manualset3
213632	2	419599	7	NULL	NULL	0	NULL	mass ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In regard to the mass ratio , although the mass ratio of calcium to phosphorus was almost constant , the mass ratios of magnesium to calcium and phosphorus were different at early and advanced stages of the accumulation of calcium and phosphorus .
	manualset3
213633	3	419599	7	NULL	NULL	0	NULL	calcium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In regard to the mass ratio , although the mass ratio of calcium to phosphorus was almost constant , the mass ratios of magnesium to calcium and phosphorus were different at early and advanced stages of the accumulation of calcium and phosphorus .
	manualset3
213634	4	419599	7	NULL	NULL	0	NULL	phosphorus	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In regard to the mass ratio , although the mass ratio of calcium to phosphorus was almost constant , the mass ratios of magnesium to calcium and phosphorus were different at early and advanced stages of the accumulation of calcium and phosphorus .
	manualset3
213635	5	419599	7	NULL	NULL	0	NULL	 mass ratios	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In regard to the mass ratio , although the mass ratio of calcium to phosphorus was almost constant , the mass ratios of magnesium to calcium and phosphorus were different at early and advanced stages of the accumulation of calcium and phosphorus .
	manualset3
213636	6	419599	7	NULL	NULL	0	NULL	magnesium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In regard to the mass ratio , although the mass ratio of calcium to phosphorus was almost constant , the mass ratios of magnesium to calcium and phosphorus were different at early and advanced stages of the accumulation of calcium and phosphorus .
	manualset3
213637	7	419599	7	NULL	NULL	0	NULL	calcium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In regard to the mass ratio , although the mass ratio of calcium to phosphorus was almost constant , the mass ratios of magnesium to calcium and phosphorus were different at early and advanced stages of the accumulation of calcium and phosphorus .
	manualset3
213638	8	419599	7	NULL	NULL	0	NULL	phosphorus 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In regard to the mass ratio , although the mass ratio of calcium to phosphorus was almost constant , the mass ratios of magnesium to calcium and phosphorus were different at early and advanced stages of the accumulation of calcium and phosphorus .
	manualset3
213639	9	419599	7	NULL	NULL	0	NULL	early stages	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In regard to the mass ratio , although the mass ratio of calcium to phosphorus was almost constant , the mass ratios of magnesium to calcium and phosphorus were different at early and advanced stages of the accumulation of calcium and phosphorus .
	manualset3
213640	10	419599	7	NULL	NULL	0	NULL	advanced stages	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In regard to the mass ratio , although the mass ratio of calcium to phosphorus was almost constant , the mass ratios of magnesium to calcium and phosphorus were different at early and advanced stages of the accumulation of calcium and phosphorus .
	manualset3
213641	11	419599	7	NULL	NULL	0	NULL	accumulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In regard to the mass ratio , although the mass ratio of calcium to phosphorus was almost constant , the mass ratios of magnesium to calcium and phosphorus were different at early and advanced stages of the accumulation of calcium and phosphorus .
	manualset3
213642	12	419599	7	NULL	NULL	0	NULL	calcium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In regard to the mass ratio , although the mass ratio of calcium to phosphorus was almost constant , the mass ratios of magnesium to calcium and phosphorus were different at early and advanced stages of the accumulation of calcium and phosphorus .
	manualset3
213643	13	419599	7	NULL	NULL	0	NULL	phosphorus	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In regard to the mass ratio , although the mass ratio of calcium to phosphorus was almost constant , the mass ratios of magnesium to calcium and phosphorus were different at early and advanced stages of the accumulation of calcium and phosphorus .
	manualset3
213644	1	419600	7	NULL	NULL	0	NULL	knowledge	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although our knowledge of craniofacial growth has increased during recent times , it is still incomplete with regard to the explanation for the regulation of craniofacial growth .
	manualset3
213645	2	419600	7	NULL	NULL	0	NULL	craniofacial growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although our knowledge of craniofacial growth has increased during recent times , it is still incomplete with regard to the explanation for the regulation of craniofacial growth .
	manualset3
213646	3	419600	7	NULL	NULL	0	NULL	recent times	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Although our knowledge of craniofacial growth has increased during recent times , it is still incomplete with regard to the explanation for the regulation of craniofacial growth .
	manualset3
213647	4	419600	7	NULL	NULL	0	NULL	explanation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although our knowledge of craniofacial growth has increased during recent times , it is still incomplete with regard to the explanation for the regulation of craniofacial growth .
	manualset3
213648	5	419600	7	NULL	NULL	0	NULL	regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although our knowledge of craniofacial growth has increased during recent times , it is still incomplete with regard to the explanation for the regulation of craniofacial growth .
	manualset3
213649	6	419600	7	NULL	NULL	0	NULL	craniofacial growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although our knowledge of craniofacial growth has increased during recent times , it is still incomplete with regard to the explanation for the regulation of craniofacial growth .
	manualset3
213650	1	419601	7	NULL	NULL	0	NULL	Proteomics 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteomics , the study of protein function within biologic systems , will further our understanding of cancer pathogenesis .
	manualset3
213651	2	419601	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteomics , the study of protein function within biologic systems , will further our understanding of cancer pathogenesis .
	manualset3
213652	3	419601	7	NULL	NULL	0	NULL	protein function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteomics , the study of protein function within biologic systems , will further our understanding of cancer pathogenesis .
	manualset3
213653	4	419601	7	NULL	NULL	NULL	NULL	biologic systems	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Proteomics , the study of protein function within biologic systems , will further our understanding of cancer pathogenesis .
	manualset3
213654	5	419601	7	NULL	NULL	0	NULL	understanding 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteomics , the study of protein function within biologic systems , will further our understanding of cancer pathogenesis .
	manualset3
213655	6	419601	7	NULL	NULL	0	NULL	cancer pathogenesis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteomics , the study of protein function within biologic systems , will further our understanding of cancer pathogenesis .
	manualset3
213656	1	419602	7	NULL	NULL	0	NULL	Natural fluorescence	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural fluorescence of collagen is due to collagen cross-linking molecules that connect single collagen fibers and therefore provide rigidity of the cervical stroma .
	manualset3
213657	2	419602	7	NULL	NULL	0	NULL	collagen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural fluorescence of collagen is due to collagen cross-linking molecules that connect single collagen fibers and therefore provide rigidity of the cervical stroma .
	manualset3
213658	3	419602	7	NULL	NULL	0	NULL	collagen cross-linking molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural fluorescence of collagen is due to collagen cross-linking molecules that connect single collagen fibers and therefore provide rigidity of the cervical stroma .
	manualset3
213659	4	419602	7	NULL	NULL	0	NULL	single collagen fibers	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural fluorescence of collagen is due to collagen cross-linking molecules that connect single collagen fibers and therefore provide rigidity of the cervical stroma .
	manualset3
213660	5	419602	7	NULL	NULL	0	NULL	rigidity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural fluorescence of collagen is due to collagen cross-linking molecules that connect single collagen fibers and therefore provide rigidity of the cervical stroma .
	manualset3
213661	6	419602	7	NULL	NULL	0	NULL	cervical stroma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Natural fluorescence of collagen is due to collagen cross-linking molecules that connect single collagen fibers and therefore provide rigidity of the cervical stroma .
	manualset3
213662	1	419603	7	NULL	NULL	NULL	NULL	Energy status	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Energy status , growth and nitrogenase activity in continuous cultures of Rhizobium sp .
	manualset3
213663	2	419603	7	NULL	NULL	NULL	NULL	growth	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Energy status , growth and nitrogenase activity in continuous cultures of Rhizobium sp .
	manualset3
213664	3	419603	7	NULL	NULL	0	NULL	nitrogenase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Energy status , growth and nitrogenase activity in continuous cultures of Rhizobium sp .
	manualset3
213665	4	419603	7	NULL	NULL	0	NULL	continuous cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Energy status , growth and nitrogenase activity in continuous cultures of Rhizobium sp .
	manualset3
213666	5	419603	7	NULL	NULL	0	NULL	Rhizobium sp	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Energy status , growth and nitrogenase activity in continuous cultures of Rhizobium sp .
	manualset3
213667	1	419604	7	NULL	NULL	0	NULL	commentary	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Note that the commentary by the author is in italics after the bibliographic information .
	manualset3
213668	2	419604	7	NULL	NULL	0	NULL	author	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Note that the commentary by the author is in italics after the bibliographic information .
	manualset3
213669	3	419604	7	NULL	NULL	0	NULL	italics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Note that the commentary by the author is in italics after the bibliographic information .
	manualset3
213670	4	419604	7	NULL	NULL	0	NULL	bibliographic information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Note that the commentary by the author is in italics after the bibliographic information .
	manualset3
213671	1	419605	7	NULL	NULL	0	NULL	attractive property`	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An attractive property of Lamb waves is that they can provide a much higher value of Deltav/v than is possible with surface acoustic waves .
	manualset3
213672	2	419605	7	NULL	NULL	0	NULL	Lamb waves	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	An attractive property of Lamb waves is that they can provide a much higher value of Deltav/v than is possible with surface acoustic waves .
	manualset3
213673	3	419605	7	NULL	NULL	0	NULL	higher value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An attractive property of Lamb waves is that they can provide a much higher value of Deltav/v than is possible with surface acoustic waves .
	manualset3
213674	4	419605	7	NULL	NULL	0	NULL	Deltav/v	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An attractive property of Lamb waves is that they can provide a much higher value of Deltav/v than is possible with surface acoustic waves .
	manualset3
213675	5	419605	7	NULL	NULL	0	NULL	surface acoustic waves	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	An attractive property of Lamb waves is that they can provide a much higher value of Deltav/v than is possible with surface acoustic waves .
	manualset3
213711	1	419606	7	NULL	NULL	0	NULL	conclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , whilst UA cooling inhibits breathing and decreases UA resistances , UA CO2 has minimal effects .
	manualset3
213712	2	419606	7	NULL	NULL	0	NULL	UA cooling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , whilst UA cooling inhibits breathing and decreases UA resistances , UA CO2 has minimal effects .
	manualset3
213713	3	419606	7	NULL	NULL	0	NULL	breathing 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , whilst UA cooling inhibits breathing and decreases UA resistances , UA CO2 has minimal effects .
	manualset3
213715	4	419606	7	NULL	NULL	0	NULL	UA resistances	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , whilst UA cooling inhibits breathing and decreases UA resistances , UA CO2 has minimal effects .
	manualset3
213716	5	419606	7	NULL	NULL	0	NULL	UA CO2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , whilst UA cooling inhibits breathing and decreases UA resistances , UA CO2 has minimal effects .
	manualset3
213717	6	419606	7	NULL	NULL	0	NULL	minimal effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , whilst UA cooling inhibits breathing and decreases UA resistances , UA CO2 has minimal effects .
	manualset3
213727	1	419607	7	NULL	NULL	0	NULL	morbidity rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The morbidity rate in patients with R0-remnant under 0.05 mmoles was 100 % , and the rate decreased in inverse proportion to R0-remnant .
	manualset3
213728	2	419607	7	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The morbidity rate in patients with R0-remnant under 0.05 mmoles was 100 % , and the rate decreased in inverse proportion to R0-remnant .
	manualset3
213729	3	419607	7	NULL	NULL	0	NULL	R0-remnant	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The morbidity rate in patients with R0-remnant under 0.05 mmoles was 100 % , and the rate decreased in inverse proportion to R0-remnant .
	manualset3
213730	4	419607	7	NULL	NULL	0	NULL	0.05 mmoles	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The morbidity rate in patients with R0-remnant under 0.05 mmoles was 100 % , and the rate decreased in inverse proportion to R0-remnant .
	manualset3
213731	5	419607	7	NULL	NULL	0	NULL	100 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The morbidity rate in patients with R0-remnant under 0.05 mmoles was 100 % , and the rate decreased in inverse proportion to R0-remnant .
	manualset3
213732	6	419607	7	NULL	NULL	0	NULL	rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The morbidity rate in patients with R0-remnant under 0.05 mmoles was 100 % , and the rate decreased in inverse proportion to R0-remnant .
	manualset3
213733	7	419607	7	NULL	NULL	0	NULL	 inverse proportion 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The morbidity rate in patients with R0-remnant under 0.05 mmoles was 100 % , and the rate decreased in inverse proportion to R0-remnant .
	manualset3
213736	8	419607	7	NULL	NULL	0	NULL	R0-remnant	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The morbidity rate in patients with R0-remnant under 0.05 mmoles was 100 % , and the rate decreased in inverse proportion to R0-remnant .
	manualset3
213742	1	419608	7	NULL	NULL	0	NULL	RNA profiles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	RNA profiles of rat olfactory epithelia : individual and age related variations .
	manualset3
213745	2	419608	7	NULL	NULL	0	NULL	 rat olfactory epithelia	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	RNA profiles of rat olfactory epithelia : individual and age related variations .
	manualset3
213747	3	419608	7	NULL	NULL	0	NULL	individual variations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	RNA profiles of rat olfactory epithelia : individual and age related variations .
	manualset3
213748	4	419608	7	NULL	NULL	0	NULL	age related variations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	RNA profiles of rat olfactory epithelia : individual and age related variations .
	manualset3
213752	1	419609	7	NULL	NULL	0	NULL	 immunoreactivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunoreactivity was confined to the cell nucleus .
	manualset3
213754	2	419609	7	NULL	NULL	0	NULL	cell nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunoreactivity was confined to the cell nucleus .
	manualset3
213755	1	419610	7	NULL	NULL	0	NULL	Cellular migration 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cellular migration and axonal outgrowth from adult mammalian peripheral nerves in vitro .
	manualset3
213756	2	419610	7	NULL	NULL	0	NULL	axonal outgrowth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cellular migration and axonal outgrowth from adult mammalian peripheral nerves in vitro .
	manualset3
213757	3	419610	7	NULL	NULL	0	NULL	adult mammalian peripheral nerves	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Cellular migration and axonal outgrowth from adult mammalian peripheral nerves in vitro .
	manualset3
213761	1	419611	7	NULL	NULL	0	NULL	parental psychological control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although parental psychological control was negatively related to adolescent psychological well-being , parental behavioral control was positively related to adolescent adjustment .
	manualset3
213770	2	419611	7	NULL	NULL	0	NULL	adolescent psychological well-being	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although parental psychological control was negatively related to adolescent psychological well-being , parental behavioral control was positively related to adolescent adjustment .
	manualset3
213775	3	419611	7	NULL	NULL	0	NULL	parental behavioral control	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although parental psychological control was negatively related to adolescent psychological well-being , parental behavioral control was positively related to adolescent adjustment .
	manualset3
213784	4	419611	7	NULL	NULL	0	NULL	adolescent adjustment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although parental psychological control was negatively related to adolescent psychological well-being , parental behavioral control was positively related to adolescent adjustment .
	manualset3
213789	1	419612	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , a Streptomyces strain producing both ePL and gPGA was identified .
	manualset3
213790	2	419612	7	NULL	NULL	0	NULL	Streptomyces strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , a Streptomyces strain producing both ePL and gPGA was identified .
	manualset3
213791	3	419612	7	NULL	NULL	0	NULL	ePL 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , a Streptomyces strain producing both ePL and gPGA was identified .
	manualset3
213792	4	419612	7	NULL	NULL	0	NULL	gPGA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , a Streptomyces strain producing both ePL and gPGA was identified .
	manualset3
213803	1	419613	7	NULL	NULL	0	NULL	 polyQ diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The polyQ diseases , including Huntington 's disease and various spinocerebellar ataxias , are caused by abnormal expansions of the polyQ stretch ( & gt ; 35-40 ) within disease-causative proteins .
	manualset3
213804	2	419613	7	NULL	NULL	0	NULL	Huntington 's disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The polyQ diseases , including Huntington 's disease and various spinocerebellar ataxias , are caused by abnormal expansions of the polyQ stretch ( & gt ; 35-40 ) within disease-causative proteins .
	manualset3
213830	3	419613	7	NULL	NULL	0	NULL	spinocerebellar ataxias	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The polyQ diseases , including Huntington 's disease and various spinocerebellar ataxias , are caused by abnormal expansions of the polyQ stretch ( & gt ; 35-40 ) within disease-causative proteins .
	manualset3
213831	4	419613	7	NULL	NULL	0	NULL	abnormal expansions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The polyQ diseases , including Huntington 's disease and various spinocerebellar ataxias , are caused by abnormal expansions of the polyQ stretch ( & gt ; 35-40 ) within disease-causative proteins .
	manualset3
213832	5	419613	7	NULL	NULL	0	NULL	polyQ stretch 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The polyQ diseases , including Huntington 's disease and various spinocerebellar ataxias , are caused by abnormal expansions of the polyQ stretch ( & gt ; 35-40 ) within disease-causative proteins .
	manualset3
213833	6	419613	7	NULL	NULL	0	NULL	& gt ; 35-40	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The polyQ diseases , including Huntington 's disease and various spinocerebellar ataxias , are caused by abnormal expansions of the polyQ stretch ( & gt ; 35-40 ) within disease-causative proteins .
	manualset3
213834	7	419613	7	NULL	NULL	0	NULL	disease-causative proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The polyQ diseases , including Huntington 's disease and various spinocerebellar ataxias , are caused by abnormal expansions of the polyQ stretch ( & gt ; 35-40 ) within disease-causative proteins .
	manualset3
213842	1	419614	7	NULL	NULL	0	NULL	Bax	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , Bax is indispensable for this type of necrosis .
	manualset3
213845	2	419614	7	NULL	NULL	0	NULL	necrosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , Bax is indispensable for this type of necrosis .
	manualset3
213853	1	419615	7	NULL	NULL	0	NULL	visual acuity levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	At all visual acuity levels , the patients ' foveal thresholds were significantly higher than those of 20 similarly aged normal observers ; threshold elevations tended to be greater for a 500-nm than for a 655-nm test flash .
	manualset3
213855	2	419615	7	NULL	NULL	0	NULL	patients ' foveal thresholds	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	At all visual acuity levels , the patients ' foveal thresholds were significantly higher than those of 20 similarly aged normal observers ; threshold elevations tended to be greater for a 500-nm than for a 655-nm test flash .
	manualset3
213856	3	419615	7	NULL	NULL	0	NULL	20 similarly aged normal observers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	At all visual acuity levels , the patients ' foveal thresholds were significantly higher than those of 20 similarly aged normal observers ; threshold elevations tended to be greater for a 500-nm than for a 655-nm test flash .
	manualset3
213865	4	419615	7	NULL	NULL	0	NULL	threshold elevations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	At all visual acuity levels , the patients ' foveal thresholds were significantly higher than those of 20 similarly aged normal observers ; threshold elevations tended to be greater for a 500-nm than for a 655-nm test flash .
	manualset3
213866	5	419615	7	NULL	NULL	0	NULL	500-nm 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	At all visual acuity levels , the patients ' foveal thresholds were significantly higher than those of 20 similarly aged normal observers ; threshold elevations tended to be greater for a 500-nm than for a 655-nm test flash .
	manualset3
213867	6	419615	7	NULL	NULL	0	NULL	655-nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	At all visual acuity levels , the patients ' foveal thresholds were significantly higher than those of 20 similarly aged normal observers ; threshold elevations tended to be greater for a 500-nm than for a 655-nm test flash .
	manualset3
213868	7	419615	7	NULL	NULL	NULL	NULL	test flash	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At all visual acuity levels , the patients ' foveal thresholds were significantly higher than those of 20 similarly aged normal observers ; threshold elevations tended to be greater for a 500-nm than for a 655-nm test flash .
	manualset3
213869	1	419616	7	NULL	NULL	0	NULL	 CD29 expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , CD29 and mvCD36 expression should be evaluated in relation to the intravascular growth pattern of lymphoma cells .
	manualset3
213870	2	419616	7	NULL	NULL	0	NULL	mvCD36 expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , CD29 and mvCD36 expression should be evaluated in relation to the intravascular growth pattern of lymphoma cells .
	manualset3
213871	3	419616	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , CD29 and mvCD36 expression should be evaluated in relation to the intravascular growth pattern of lymphoma cells .
	manualset3
213872	4	419616	7	NULL	NULL	0	NULL	 intravascular growth pattern 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , CD29 and mvCD36 expression should be evaluated in relation to the intravascular growth pattern of lymphoma cells .
	manualset3
213873	5	419616	7	NULL	NULL	0	NULL	lymphoma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , CD29 and mvCD36 expression should be evaluated in relation to the intravascular growth pattern of lymphoma cells .
	manualset3
213874	1	419617	7	NULL	NULL	0	NULL	Double reciprocal analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Double reciprocal or Scatchard plot analysis indicates that the binding of Ac-Phe-tRNAPhe to the ribosomal sites is a cooperative process .
	manualset3
213875	2	419617	7	NULL	NULL	0	NULL	Scatchard plot analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Double reciprocal or Scatchard plot analysis indicates that the binding of Ac-Phe-tRNAPhe to the ribosomal sites is a cooperative process .
	manualset3
213876	3	419617	7	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Double reciprocal or Scatchard plot analysis indicates that the binding of Ac-Phe-tRNAPhe to the ribosomal sites is a cooperative process .
	manualset3
213877	4	419617	7	NULL	NULL	0	NULL	Ac-Phe-tRNAPhe	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Double reciprocal or Scatchard plot analysis indicates that the binding of Ac-Phe-tRNAPhe to the ribosomal sites is a cooperative process .
	manualset3
213878	5	419617	7	NULL	NULL	0	NULL	ribosomal sites	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Double reciprocal or Scatchard plot analysis indicates that the binding of Ac-Phe-tRNAPhe to the ribosomal sites is a cooperative process .
	manualset3
213879	6	419617	7	NULL	NULL	NULL	NULL	cooperative process	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Double reciprocal or Scatchard plot analysis indicates that the binding of Ac-Phe-tRNAPhe to the ribosomal sites is a cooperative process .
	manualset3
213880	1	419618	7	NULL	NULL	0	NULL	Eight patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Eight patients regenerated hyaline cartilage and also contained type-X collagen in the deepest layers and type-II collagen in the deep layers .
	manualset3
213881	2	419618	7	NULL	NULL	NULL	NULL	hyaline cartilage 	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Eight patients regenerated hyaline cartilage and also contained type-X collagen in the deepest layers and type-II collagen in the deep layers .
	manualset3
213882	3	419618	7	NULL	NULL	0	NULL	type-X collagen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Eight patients regenerated hyaline cartilage and also contained type-X collagen in the deepest layers and type-II collagen in the deep layers .
	manualset3
213883	4	419618	7	NULL	NULL	0	NULL	deepest layers	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Eight patients regenerated hyaline cartilage and also contained type-X collagen in the deepest layers and type-II collagen in the deep layers .
	manualset3
213884	5	419618	7	NULL	NULL	NULL	NULL	type-II collagen	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Eight patients regenerated hyaline cartilage and also contained type-X collagen in the deepest layers and type-II collagen in the deep layers .
	manualset3
213885	6	419618	7	NULL	NULL	0	NULL	deep layers 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Eight patients regenerated hyaline cartilage and also contained type-X collagen in the deepest layers and type-II collagen in the deep layers .
	manualset3
213886	1	419619	7	NULL	NULL	0	NULL	Ala	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although Ala , amongst the native E. coli periplasmic proteins , is the preferred X ( +1 ) residue with an occurrence of 50 % frequency , it proved half as effective in promoting export when inserted proximally to the SS of cytochrome b ( 5 ) .
	manualset3
213887	2	419619	7	NULL	NULL	0	NULL	native E. coli periplasmic proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although Ala , amongst the native E. coli periplasmic proteins , is the preferred X ( +1 ) residue with an occurrence of 50 % frequency , it proved half as effective in promoting export when inserted proximally to the SS of cytochrome b ( 5 ) .
	manualset3
213888	3	419619	7	NULL	NULL	0	NULL	 X ( +1 ) residue	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Although Ala , amongst the native E. coli periplasmic proteins , is the preferred X ( +1 ) residue with an occurrence of 50 % frequency , it proved half as effective in promoting export when inserted proximally to the SS of cytochrome b ( 5 ) .
	manualset3
213889	4	419619	7	NULL	NULL	0	NULL	50 % frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although Ala , amongst the native E. coli periplasmic proteins , is the preferred X ( +1 ) residue with an occurrence of 50 % frequency , it proved half as effective in promoting export when inserted proximally to the SS of cytochrome b ( 5 ) .
	manualset3
213890	5	419619	7	NULL	NULL	NULL	NULL	export	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although Ala , amongst the native E. coli periplasmic proteins , is the preferred X ( +1 ) residue with an occurrence of 50 % frequency , it proved half as effective in promoting export when inserted proximally to the SS of cytochrome b ( 5 ) .
	manualset3
213891	6	419619	7	NULL	NULL	0	NULL	proximally to the SS of cytochrome b	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although Ala , amongst the native E. coli periplasmic proteins , is the preferred X ( +1 ) residue with an occurrence of 50 % frequency , it proved half as effective in promoting export when inserted proximally to the SS of cytochrome b ( 5 ) .
	manualset3
213892	1	419620	7	NULL	NULL	0	NULL	molecular mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the molecular mechanisms that limit target gene responses to specific domains are unclear .
	manualset3
213893	2	419620	7	NULL	NULL	0	NULL	gene responses	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the molecular mechanisms that limit target gene responses to specific domains are unclear .
	manualset3
213894	3	419620	7	NULL	NULL	0	NULL	domains	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the molecular mechanisms that limit target gene responses to specific domains are unclear .
	manualset3
213951	1	419621	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that both size of tissue injury and edema were reduced in the old subjects only up to 1DPL , correlating with a slower progression of neurodegeneration with peak numbers of degenerating neurons at 3DPL in the aged , contrasting with maximum neurodegeneration at 1DPL in the young .
	manualset3
213953	2	419621	7	NULL	NULL	0	NULL	 size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that both size of tissue injury and edema were reduced in the old subjects only up to 1DPL , correlating with a slower progression of neurodegeneration with peak numbers of degenerating neurons at 3DPL in the aged , contrasting with maximum neurodegeneration at 1DPL in the young .
	manualset3
213955	3	419621	7	NULL	NULL	0	NULL	tissue injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that both size of tissue injury and edema were reduced in the old subjects only up to 1DPL , correlating with a slower progression of neurodegeneration with peak numbers of degenerating neurons at 3DPL in the aged , contrasting with maximum neurodegeneration at 1DPL in the young .
	manualset3
213957	4	419621	7	NULL	NULL	0	NULL	edema	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that both size of tissue injury and edema were reduced in the old subjects only up to 1DPL , correlating with a slower progression of neurodegeneration with peak numbers of degenerating neurons at 3DPL in the aged , contrasting with maximum neurodegeneration at 1DPL in the young .
	manualset3
213958	5	419621	7	NULL	NULL	0	NULL	old subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that both size of tissue injury and edema were reduced in the old subjects only up to 1DPL , correlating with a slower progression of neurodegeneration with peak numbers of degenerating neurons at 3DPL in the aged , contrasting with maximum neurodegeneration at 1DPL in the young .
	manualset3
213981	6	419621	7	NULL	NULL	0	NULL	1DPL	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that both size of tissue injury and edema were reduced in the old subjects only up to 1DPL , correlating with a slower progression of neurodegeneration with peak numbers of degenerating neurons at 3DPL in the aged , contrasting with maximum neurodegeneration at 1DPL in the young .
	manualset3
213983	7	419621	7	NULL	NULL	0	NULL	slower progression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that both size of tissue injury and edema were reduced in the old subjects only up to 1DPL , correlating with a slower progression of neurodegeneration with peak numbers of degenerating neurons at 3DPL in the aged , contrasting with maximum neurodegeneration at 1DPL in the young .
	manualset3
213984	8	419621	7	NULL	NULL	0	NULL	neurodegeneration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that both size of tissue injury and edema were reduced in the old subjects only up to 1DPL , correlating with a slower progression of neurodegeneration with peak numbers of degenerating neurons at 3DPL in the aged , contrasting with maximum neurodegeneration at 1DPL in the young .
	manualset3
213985	9	419621	7	NULL	NULL	0	NULL	peak numbers 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that both size of tissue injury and edema were reduced in the old subjects only up to 1DPL , correlating with a slower progression of neurodegeneration with peak numbers of degenerating neurons at 3DPL in the aged , contrasting with maximum neurodegeneration at 1DPL in the young .
	manualset3
213986	10	419621	7	NULL	NULL	0	NULL	degenerating neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that both size of tissue injury and edema were reduced in the old subjects only up to 1DPL , correlating with a slower progression of neurodegeneration with peak numbers of degenerating neurons at 3DPL in the aged , contrasting with maximum neurodegeneration at 1DPL in the young .
	manualset3
213987	11	419621	7	NULL	NULL	0	NULL	 3DPL	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that both size of tissue injury and edema were reduced in the old subjects only up to 1DPL , correlating with a slower progression of neurodegeneration with peak numbers of degenerating neurons at 3DPL in the aged , contrasting with maximum neurodegeneration at 1DPL in the young .
	manualset3
213988	12	419621	7	NULL	NULL	0	NULL	maximum neurodegeneration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that both size of tissue injury and edema were reduced in the old subjects only up to 1DPL , correlating with a slower progression of neurodegeneration with peak numbers of degenerating neurons at 3DPL in the aged , contrasting with maximum neurodegeneration at 1DPL in the young .
	manualset3
213989	13	419621	7	NULL	NULL	0	NULL	1DPL	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that both size of tissue injury and edema were reduced in the old subjects only up to 1DPL , correlating with a slower progression of neurodegeneration with peak numbers of degenerating neurons at 3DPL in the aged , contrasting with maximum neurodegeneration at 1DPL in the young .
	manualset3
213990	14	419621	7	NULL	NULL	0	NULL	young	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results show that both size of tissue injury and edema were reduced in the old subjects only up to 1DPL , correlating with a slower progression of neurodegeneration with peak numbers of degenerating neurons at 3DPL in the aged , contrasting with maximum neurodegeneration at 1DPL in the young .
	manualset3
213991	1	419622	7	NULL	NULL	0	NULL	thecal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	For thecal cells of large follicles , LH increased ( p & lt ; 0.01 ) GJIC , whereas FSH or LH + FSH had no effects .
	manualset3
213992	2	419622	7	NULL	NULL	0	NULL	large follicles	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	For thecal cells of large follicles , LH increased ( p & lt ; 0.01 ) GJIC , whereas FSH or LH + FSH had no effects .
	manualset3
213993	3	419622	7	NULL	NULL	0	NULL	LH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For thecal cells of large follicles , LH increased ( p & lt ; 0.01 ) GJIC , whereas FSH or LH + FSH had no effects .
	manualset3
213994	4	419622	7	NULL	NULL	0	NULL	p & lt ; 0.01	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For thecal cells of large follicles , LH increased ( p & lt ; 0.01 ) GJIC , whereas FSH or LH + FSH had no effects .
	manualset3
213995	5	419622	7	NULL	NULL	0	NULL	GJIC	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For thecal cells of large follicles , LH increased ( p & lt ; 0.01 ) GJIC , whereas FSH or LH + FSH had no effects .
	manualset3
213996	6	419622	7	NULL	NULL	0	NULL	FSH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For thecal cells of large follicles , LH increased ( p & lt ; 0.01 ) GJIC , whereas FSH or LH + FSH had no effects .
	manualset3
213997	7	419622	7	NULL	NULL	0	NULL	LH + FSH 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For thecal cells of large follicles , LH increased ( p & lt ; 0.01 ) GJIC , whereas FSH or LH + FSH had no effects .
	manualset3
214851	8	419622	7	NULL	NULL	0	NULL	no effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For thecal cells of large follicles , LH increased ( p & lt ; 0.01 ) GJIC , whereas FSH or LH + FSH had no effects .
	manualset3
213998	1	419623	7	NULL	NULL	NULL	NULL	adrenal medullary chromaffin cells  ( AMCC )	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The adrenal medullary chromaffin cells ( AMCC ) transition to the neuronal phenotype is known to occur in asthma , as evidenced by degranulation of chromaffin granules , decline of epinephrine ( EPI ) and phenylethanolamine-n-methyl transferase ( PNMT ) , and obvious alterations in cellular architecture .
	manualset3
214000	3	419623	7	NULL	NULL	NULL	NULL	neuronal phenotype	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The adrenal medullary chromaffin cells ( AMCC ) transition to the neuronal phenotype is known to occur in asthma , as evidenced by degranulation of chromaffin granules , decline of epinephrine ( EPI ) and phenylethanolamine-n-methyl transferase ( PNMT ) , and obvious alterations in cellular architecture .
	manualset3
214001	4	419623	7	NULL	NULL	0	NULL	asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The adrenal medullary chromaffin cells ( AMCC ) transition to the neuronal phenotype is known to occur in asthma , as evidenced by degranulation of chromaffin granules , decline of epinephrine ( EPI ) and phenylethanolamine-n-methyl transferase ( PNMT ) , and obvious alterations in cellular architecture .
	manualset3
214002	5	419623	7	NULL	NULL	NULL	NULL	 degranulation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The adrenal medullary chromaffin cells ( AMCC ) transition to the neuronal phenotype is known to occur in asthma , as evidenced by degranulation of chromaffin granules , decline of epinephrine ( EPI ) and phenylethanolamine-n-methyl transferase ( PNMT ) , and obvious alterations in cellular architecture .
	manualset3
214003	6	419623	7	NULL	NULL	NULL	NULL	chromaffin granules	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The adrenal medullary chromaffin cells ( AMCC ) transition to the neuronal phenotype is known to occur in asthma , as evidenced by degranulation of chromaffin granules , decline of epinephrine ( EPI ) and phenylethanolamine-n-methyl transferase ( PNMT ) , and obvious alterations in cellular architecture .
	manualset3
214004	7	419623	7	NULL	NULL	0	NULL	decline 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The adrenal medullary chromaffin cells ( AMCC ) transition to the neuronal phenotype is known to occur in asthma , as evidenced by degranulation of chromaffin granules , decline of epinephrine ( EPI ) and phenylethanolamine-n-methyl transferase ( PNMT ) , and obvious alterations in cellular architecture .
	manualset3
214005	8	419623	7	NULL	NULL	0	NULL	epinephrine ( EPI )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The adrenal medullary chromaffin cells ( AMCC ) transition to the neuronal phenotype is known to occur in asthma , as evidenced by degranulation of chromaffin granules , decline of epinephrine ( EPI ) and phenylethanolamine-n-methyl transferase ( PNMT ) , and obvious alterations in cellular architecture .
	manualset3
214006	9	419623	7	NULL	NULL	0	NULL	phenylethanolamine-n-methyl transferase ( PNMT )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The adrenal medullary chromaffin cells ( AMCC ) transition to the neuronal phenotype is known to occur in asthma , as evidenced by degranulation of chromaffin granules , decline of epinephrine ( EPI ) and phenylethanolamine-n-methyl transferase ( PNMT ) , and obvious alterations in cellular architecture .
	manualset3
214007	10	419623	7	NULL	NULL	0	NULL	alterations 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The adrenal medullary chromaffin cells ( AMCC ) transition to the neuronal phenotype is known to occur in asthma , as evidenced by degranulation of chromaffin granules , decline of epinephrine ( EPI ) and phenylethanolamine-n-methyl transferase ( PNMT ) , and obvious alterations in cellular architecture .
	manualset3
214008	11	419623	7	NULL	NULL	NULL	NULL	cellular architecture 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The adrenal medullary chromaffin cells ( AMCC ) transition to the neuronal phenotype is known to occur in asthma , as evidenced by degranulation of chromaffin granules , decline of epinephrine ( EPI ) and phenylethanolamine-n-methyl transferase ( PNMT ) , and obvious alterations in cellular architecture .
	manualset3
215150	12	419623	7	NULL	NULL	0	NULL	transition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The adrenal medullary chromaffin cells ( AMCC ) transition to the neuronal phenotype is known to occur in asthma , as evidenced by degranulation of chromaffin granules , decline of epinephrine ( EPI ) and phenylethanolamine-n-methyl transferase ( PNMT ) , and obvious alterations in cellular architecture .
	manualset3
214009	1	419624	7	NULL	NULL	0	NULL	protein kinase C ( PK-C ) activator	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Both the protein kinase C ( PK-C ) activator , phorbol 12-myristate 13-acetate ( PMA ) , and the cyclic AMP-dependent protein kinase ( PK-A ) activator , 8-bromo-cyclic AMP ( 8-BR ) , have been shown to increase 32P incorporation into glial fibrillary acidic protein ( GFAP ) and vimentin in cultured astrocytes .
	manualset3
214010	2	419624	7	NULL	NULL	0	NULL	phorbol 12-myristate 13-acetate ( PMA ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Both the protein kinase C ( PK-C ) activator , phorbol 12-myristate 13-acetate ( PMA ) , and the cyclic AMP-dependent protein kinase ( PK-A ) activator , 8-bromo-cyclic AMP ( 8-BR ) , have been shown to increase 32P incorporation into glial fibrillary acidic protein ( GFAP ) and vimentin in cultured astrocytes .
	manualset3
214011	3	419624	7	NULL	NULL	0	NULL	cyclic AMP-dependent protein kinase ( PK-A ) activator	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Both the protein kinase C ( PK-C ) activator , phorbol 12-myristate 13-acetate ( PMA ) , and the cyclic AMP-dependent protein kinase ( PK-A ) activator , 8-bromo-cyclic AMP ( 8-BR ) , have been shown to increase 32P incorporation into glial fibrillary acidic protein ( GFAP ) and vimentin in cultured astrocytes .
	manualset3
214012	4	419624	7	NULL	NULL	0	NULL	8-bromo-cyclic AMP ( 8-BR )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Both the protein kinase C ( PK-C ) activator , phorbol 12-myristate 13-acetate ( PMA ) , and the cyclic AMP-dependent protein kinase ( PK-A ) activator , 8-bromo-cyclic AMP ( 8-BR ) , have been shown to increase 32P incorporation into glial fibrillary acidic protein ( GFAP ) and vimentin in cultured astrocytes .
	manualset3
214013	5	419624	7	NULL	NULL	0	NULL	32P incorporation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Both the protein kinase C ( PK-C ) activator , phorbol 12-myristate 13-acetate ( PMA ) , and the cyclic AMP-dependent protein kinase ( PK-A ) activator , 8-bromo-cyclic AMP ( 8-BR ) , have been shown to increase 32P incorporation into glial fibrillary acidic protein ( GFAP ) and vimentin in cultured astrocytes .
	manualset3
214014	6	419624	7	NULL	NULL	0	NULL	glial fibrillary acidic protein ( GFAP ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Both the protein kinase C ( PK-C ) activator , phorbol 12-myristate 13-acetate ( PMA ) , and the cyclic AMP-dependent protein kinase ( PK-A ) activator , 8-bromo-cyclic AMP ( 8-BR ) , have been shown to increase 32P incorporation into glial fibrillary acidic protein ( GFAP ) and vimentin in cultured astrocytes .
	manualset3
214015	7	419624	7	NULL	NULL	0	NULL	vimentin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Both the protein kinase C ( PK-C ) activator , phorbol 12-myristate 13-acetate ( PMA ) , and the cyclic AMP-dependent protein kinase ( PK-A ) activator , 8-bromo-cyclic AMP ( 8-BR ) , have been shown to increase 32P incorporation into glial fibrillary acidic protein ( GFAP ) and vimentin in cultured astrocytes .
	manualset3
214016	8	419624	7	NULL	NULL	0	NULL	cultured astrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Both the protein kinase C ( PK-C ) activator , phorbol 12-myristate 13-acetate ( PMA ) , and the cyclic AMP-dependent protein kinase ( PK-A ) activator , 8-bromo-cyclic AMP ( 8-BR ) , have been shown to increase 32P incorporation into glial fibrillary acidic protein ( GFAP ) and vimentin in cultured astrocytes .
	manualset3
214017	1	419625	7	NULL	NULL	0	NULL	Hairless rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hairless rats were exposed to a potent topical corticosteroid ( Temovate ) in combination with either DMSO alone or with PADMA 28 given topically .
	manualset3
214018	2	419625	7	NULL	NULL	0	NULL	topical corticosteroid	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Hairless rats were exposed to a potent topical corticosteroid ( Temovate ) in combination with either DMSO alone or with PADMA 28 given topically .
	manualset3
214019	3	419625	7	NULL	NULL	0	NULL	Temovate	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Hairless rats were exposed to a potent topical corticosteroid ( Temovate ) in combination with either DMSO alone or with PADMA 28 given topically .
	manualset3
214020	4	419625	7	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Hairless rats were exposed to a potent topical corticosteroid ( Temovate ) in combination with either DMSO alone or with PADMA 28 given topically .
	manualset3
214021	5	419625	7	NULL	NULL	0	NULL	DMSO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Hairless rats were exposed to a potent topical corticosteroid ( Temovate ) in combination with either DMSO alone or with PADMA 28 given topically .
	manualset3
214022	6	419625	7	NULL	NULL	0	NULL	PADMA 28	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Hairless rats were exposed to a potent topical corticosteroid ( Temovate ) in combination with either DMSO alone or with PADMA 28 given topically .
	manualset3
214023	1	419626	7	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of this methylation pathway is decreased upon stimulation of platelets by various agonists .
	manualset3
214024	2	419626	7	NULL	NULL	0	NULL	methylation pathway 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of this methylation pathway is decreased upon stimulation of platelets by various agonists .
	manualset3
214025	3	419626	7	NULL	NULL	0	NULL	stimulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of this methylation pathway is decreased upon stimulation of platelets by various agonists .
	manualset3
214026	4	419626	7	NULL	NULL	0	NULL	platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of this methylation pathway is decreased upon stimulation of platelets by various agonists .
	manualset3
214027	5	419626	7	NULL	NULL	0	NULL	agonists	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of this methylation pathway is decreased upon stimulation of platelets by various agonists .
	manualset3
214028	1	419627	7	NULL	NULL	0	NULL	prearrival trauma predicted future depression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although prearrival trauma predicted future depression , other sociodemographic characteristics assumed more importance with time .
	manualset3
214029	2	419627	7	NULL	NULL	0	NULL	sociodemographic characteristics	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Although prearrival trauma predicted future depression , other sociodemographic characteristics assumed more importance with time .
	manualset3
214030	3	419627	7	NULL	NULL	0	NULL	 time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Although prearrival trauma predicted future depression , other sociodemographic characteristics assumed more importance with time .
	manualset3
214031	1	419628	7	NULL	NULL	0	NULL	resulting structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting structures were microscopic patterns of enzyme-containing lines of a redox hydrogel with a line width of about 100 microm .
	manualset3
214032	2	419628	7	NULL	NULL	0	NULL	microscopic patterns	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting structures were microscopic patterns of enzyme-containing lines of a redox hydrogel with a line width of about 100 microm .
	manualset3
214033	3	419628	7	NULL	NULL	0	NULL	enzyme-containing lines	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting structures were microscopic patterns of enzyme-containing lines of a redox hydrogel with a line width of about 100 microm .
	manualset3
214034	4	419628	7	NULL	NULL	0	NULL	redox hydrogel	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting structures were microscopic patterns of enzyme-containing lines of a redox hydrogel with a line width of about 100 microm .
	manualset3
214035	5	419628	7	NULL	NULL	0	NULL	line width	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting structures were microscopic patterns of enzyme-containing lines of a redox hydrogel with a line width of about 100 microm .
	manualset3
214036	6	419628	7	NULL	NULL	0	NULL	100 microm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The resulting structures were microscopic patterns of enzyme-containing lines of a redox hydrogel with a line width of about 100 microm .
	manualset3
214037	1	419629	7	NULL	NULL	0	NULL	T lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , T lymphocytes differentiate and mature in the thymus and are released into the peripheral circulation , where they can travel to sites of encounter with antigen .
	manualset3
214038	2	419629	7	NULL	NULL	0	NULL	thymus	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , T lymphocytes differentiate and mature in the thymus and are released into the peripheral circulation , where they can travel to sites of encounter with antigen .
	manualset3
214039	3	419629	7	NULL	NULL	0	NULL	peripheral circulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , T lymphocytes differentiate and mature in the thymus and are released into the peripheral circulation , where they can travel to sites of encounter with antigen .
	manualset3
214040	4	419629	7	NULL	NULL	0	NULL	 travel 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , T lymphocytes differentiate and mature in the thymus and are released into the peripheral circulation , where they can travel to sites of encounter with antigen .
	manualset3
214041	5	419629	7	NULL	NULL	0	NULL	sites of encounter	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , T lymphocytes differentiate and mature in the thymus and are released into the peripheral circulation , where they can travel to sites of encounter with antigen .
	manualset3
214042	6	419629	7	NULL	NULL	0	NULL	antigen	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , T lymphocytes differentiate and mature in the thymus and are released into the peripheral circulation , where they can travel to sites of encounter with antigen .
	manualset3
214043	1	419630	7	NULL	NULL	0	NULL	biomechanical basis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The biomechanical basis for occipitoatlantal dislocation is discussed , and the author suggests that distraction , in concert with variable combinations of extension , rotation , and posterior translation is responsible for occipitoatlantal dislocations .
	manualset3
214044	2	419630	7	NULL	NULL	0	NULL	occipitoatlantal dislocation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The biomechanical basis for occipitoatlantal dislocation is discussed , and the author suggests that distraction , in concert with variable combinations of extension , rotation , and posterior translation is responsible for occipitoatlantal dislocations .
	manualset3
214045	3	419630	7	NULL	NULL	0	NULL	author	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The biomechanical basis for occipitoatlantal dislocation is discussed , and the author suggests that distraction , in concert with variable combinations of extension , rotation , and posterior translation is responsible for occipitoatlantal dislocations .
	manualset3
214046	4	419630	7	NULL	NULL	0	NULL	distraction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The biomechanical basis for occipitoatlantal dislocation is discussed , and the author suggests that distraction , in concert with variable combinations of extension , rotation , and posterior translation is responsible for occipitoatlantal dislocations .
	manualset3
214047	5	419630	7	NULL	NULL	0	NULL	variable combinations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The biomechanical basis for occipitoatlantal dislocation is discussed , and the author suggests that distraction , in concert with variable combinations of extension , rotation , and posterior translation is responsible for occipitoatlantal dislocations .
	manualset3
214048	6	419630	7	NULL	NULL	0	NULL	extension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The biomechanical basis for occipitoatlantal dislocation is discussed , and the author suggests that distraction , in concert with variable combinations of extension , rotation , and posterior translation is responsible for occipitoatlantal dislocations .
	manualset3
214049	7	419630	7	NULL	NULL	0	NULL	rotation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The biomechanical basis for occipitoatlantal dislocation is discussed , and the author suggests that distraction , in concert with variable combinations of extension , rotation , and posterior translation is responsible for occipitoatlantal dislocations .
	manualset3
214050	8	419630	7	NULL	NULL	0	NULL	posterior translation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The biomechanical basis for occipitoatlantal dislocation is discussed , and the author suggests that distraction , in concert with variable combinations of extension , rotation , and posterior translation is responsible for occipitoatlantal dislocations .
	manualset3
214051	9	419630	7	NULL	NULL	0	NULL	occipitoatlantal dislocations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The biomechanical basis for occipitoatlantal dislocation is discussed , and the author suggests that distraction , in concert with variable combinations of extension , rotation , and posterior translation is responsible for occipitoatlantal dislocations .
	manualset3
214222	1	419631	7	NULL	NULL	0	NULL	 system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The system for naming and classifying herpesviruses proposed in this memorandum is intended for consideration by other workers before a final proposal is made to the International Commission for Nomenclature of Viruses .
	manualset3
214223	2	419631	7	NULL	NULL	NULL	NULL	naming herpesviruses	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The system for naming and classifying herpesviruses proposed in this memorandum is intended for consideration by other workers before a final proposal is made to the International Commission for Nomenclature of Viruses .
	manualset3
214224	3	419631	7	NULL	NULL	0	NULL	classifying herpesviruses	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The system for naming and classifying herpesviruses proposed in this memorandum is intended for consideration by other workers before a final proposal is made to the International Commission for Nomenclature of Viruses .
	manualset3
214225	4	419631	7	NULL	NULL	0	NULL	memorandum	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The system for naming and classifying herpesviruses proposed in this memorandum is intended for consideration by other workers before a final proposal is made to the International Commission for Nomenclature of Viruses .
	manualset3
214226	5	419631	7	NULL	NULL	0	NULL	consideration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The system for naming and classifying herpesviruses proposed in this memorandum is intended for consideration by other workers before a final proposal is made to the International Commission for Nomenclature of Viruses .
	manualset3
214227	6	419631	7	NULL	NULL	0	NULL	workers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The system for naming and classifying herpesviruses proposed in this memorandum is intended for consideration by other workers before a final proposal is made to the International Commission for Nomenclature of Viruses .
	manualset3
214228	7	419631	7	NULL	NULL	0	NULL	 final proposal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The system for naming and classifying herpesviruses proposed in this memorandum is intended for consideration by other workers before a final proposal is made to the International Commission for Nomenclature of Viruses .
	manualset3
214229	8	419631	7	NULL	NULL	0	NULL	International Commission for Nomenclature of Viruses	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The system for naming and classifying herpesviruses proposed in this memorandum is intended for consideration by other workers before a final proposal is made to the International Commission for Nomenclature of Viruses .
	manualset3
214230	1	419632	7	NULL	NULL	0	NULL	Al	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Also , Al induced reproductive toxicity and exerted a significant adverse effect on the steroidogenesis .
	manualset3
214231	2	419632	7	NULL	NULL	0	NULL	 reproductive toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Also , Al induced reproductive toxicity and exerted a significant adverse effect on the steroidogenesis .
	manualset3
214232	3	419632	7	NULL	NULL	0	NULL	adverse effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Also , Al induced reproductive toxicity and exerted a significant adverse effect on the steroidogenesis .
	manualset3
214233	4	419632	7	NULL	NULL	0	NULL	steroidogenesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Also , Al induced reproductive toxicity and exerted a significant adverse effect on the steroidogenesis .
	manualset3
214234	1	419633	7	NULL	NULL	0	NULL	case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of an eight year old girl is presented who was seen because of secondary enuresis and recurrent urinary tract infection .
	manualset3
214235	2	419633	7	NULL	NULL	0	NULL	eight year old girl 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of an eight year old girl is presented who was seen because of secondary enuresis and recurrent urinary tract infection .
	manualset3
214236	3	419633	7	NULL	NULL	0	NULL	secondary enuresis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of an eight year old girl is presented who was seen because of secondary enuresis and recurrent urinary tract infection .
	manualset3
214237	4	419633	7	NULL	NULL	0	NULL	recurrent urinary tract infection	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of an eight year old girl is presented who was seen because of secondary enuresis and recurrent urinary tract infection .
	manualset3
214238	1	419634	7	NULL	NULL	0	NULL	Optimizing 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimizing the growth of stressed Helicobacter pylori .
	manualset3
214239	2	419634	7	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimizing the growth of stressed Helicobacter pylori .
	manualset3
214240	3	419634	7	NULL	NULL	0	NULL	stressed Helicobacter pylori	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Optimizing the growth of stressed Helicobacter pylori .
	manualset3
214241	1	419635	7	NULL	NULL	0	NULL	 anti-M150 Ab	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , anti-M150 Ab significantly decreased the proliferation of Th cells , MLR , and production of IFN-gamma , when macrophages were utilized to provide costimulatory signals , but not when B cells were used as APC .
	manualset3
214242	2	419635	7	NULL	NULL	0	NULL	proliferation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , anti-M150 Ab significantly decreased the proliferation of Th cells , MLR , and production of IFN-gamma , when macrophages were utilized to provide costimulatory signals , but not when B cells were used as APC .
	manualset3
214243	3	419635	7	NULL	NULL	0	NULL	Th cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , anti-M150 Ab significantly decreased the proliferation of Th cells , MLR , and production of IFN-gamma , when macrophages were utilized to provide costimulatory signals , but not when B cells were used as APC .
	manualset3
214244	4	419635	7	NULL	NULL	0	NULL	MLR	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , anti-M150 Ab significantly decreased the proliferation of Th cells , MLR , and production of IFN-gamma , when macrophages were utilized to provide costimulatory signals , but not when B cells were used as APC .
	manualset3
214245	5	419635	7	NULL	NULL	0	NULL	production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , anti-M150 Ab significantly decreased the proliferation of Th cells , MLR , and production of IFN-gamma , when macrophages were utilized to provide costimulatory signals , but not when B cells were used as APC .
	manualset3
214246	6	419635	7	NULL	NULL	0	NULL	IFN-gamma	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , anti-M150 Ab significantly decreased the proliferation of Th cells , MLR , and production of IFN-gamma , when macrophages were utilized to provide costimulatory signals , but not when B cells were used as APC .
	manualset3
214247	7	419635	7	NULL	NULL	0	NULL	macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , anti-M150 Ab significantly decreased the proliferation of Th cells , MLR , and production of IFN-gamma , when macrophages were utilized to provide costimulatory signals , but not when B cells were used as APC .
	manualset3
214248	8	419635	7	NULL	NULL	0	NULL	costimulatory signals	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , anti-M150 Ab significantly decreased the proliferation of Th cells , MLR , and production of IFN-gamma , when macrophages were utilized to provide costimulatory signals , but not when B cells were used as APC .
	manualset3
214249	9	419635	7	NULL	NULL	0	NULL	B cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , anti-M150 Ab significantly decreased the proliferation of Th cells , MLR , and production of IFN-gamma , when macrophages were utilized to provide costimulatory signals , but not when B cells were used as APC .
	manualset3
214250	10	419635	7	NULL	NULL	0	NULL	APC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , anti-M150 Ab significantly decreased the proliferation of Th cells , MLR , and production of IFN-gamma , when macrophages were utilized to provide costimulatory signals , but not when B cells were used as APC .
	manualset3
214251	1	419636	7	NULL	NULL	0	NULL	previous studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although previous studies have shown that keratinocyte Ca ( 2 + ) sequestration and fluxes are controlled by sphingolipid signaling , the role of this signaling pathway in DD previously has not been investigated .
	manualset3
214252	2	419636	7	NULL	NULL	0	NULL	 keratinocyte Ca ( 2 + ) sequestration	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although previous studies have shown that keratinocyte Ca ( 2 + ) sequestration and fluxes are controlled by sphingolipid signaling , the role of this signaling pathway in DD previously has not been investigated .
	manualset3
214253	3	419636	7	NULL	NULL	0	NULL	 fluxes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although previous studies have shown that keratinocyte Ca ( 2 + ) sequestration and fluxes are controlled by sphingolipid signaling , the role of this signaling pathway in DD previously has not been investigated .
	manualset3
214254	4	419636	7	NULL	NULL	0	NULL	sphingolipid signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although previous studies have shown that keratinocyte Ca ( 2 + ) sequestration and fluxes are controlled by sphingolipid signaling , the role of this signaling pathway in DD previously has not been investigated .
	manualset3
214255	5	419636	7	NULL	NULL	0	NULL	 role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although previous studies have shown that keratinocyte Ca ( 2 + ) sequestration and fluxes are controlled by sphingolipid signaling , the role of this signaling pathway in DD previously has not been investigated .
	manualset3
214256	6	419636	7	NULL	NULL	0	NULL	signaling pathway 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although previous studies have shown that keratinocyte Ca ( 2 + ) sequestration and fluxes are controlled by sphingolipid signaling , the role of this signaling pathway in DD previously has not been investigated .
	manualset3
214257	7	419636	7	NULL	NULL	0	NULL	DD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Although previous studies have shown that keratinocyte Ca ( 2 + ) sequestration and fluxes are controlled by sphingolipid signaling , the role of this signaling pathway in DD previously has not been investigated .
	manualset3
214258	1	419637	7	NULL	NULL	0	NULL	field	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In the field of muscle regulation , there is still controversy as to whether Ca2 + , alone , is able to shift muscle from the relaxed to the fully active state or whether cross-bridge binding also contributes to turning on muscle contraction .
	manualset3
214259	2	419637	7	NULL	NULL	0	NULL	muscle regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the field of muscle regulation , there is still controversy as to whether Ca2 + , alone , is able to shift muscle from the relaxed to the fully active state or whether cross-bridge binding also contributes to turning on muscle contraction .
	manualset3
214260	3	419637	7	NULL	NULL	0	NULL	Ca2 +	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the field of muscle regulation , there is still controversy as to whether Ca2 + , alone , is able to shift muscle from the relaxed to the fully active state or whether cross-bridge binding also contributes to turning on muscle contraction .
	manualset3
214261	4	419637	7	NULL	NULL	0	NULL	 muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the field of muscle regulation , there is still controversy as to whether Ca2 + , alone , is able to shift muscle from the relaxed to the fully active state or whether cross-bridge binding also contributes to turning on muscle contraction .
	manualset3
214262	5	419637	7	NULL	NULL	0	NULL	fully active state	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the field of muscle regulation , there is still controversy as to whether Ca2 + , alone , is able to shift muscle from the relaxed to the fully active state or whether cross-bridge binding also contributes to turning on muscle contraction .
	manualset3
214263	6	419637	7	NULL	NULL	0	NULL	cross-bridge binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the field of muscle regulation , there is still controversy as to whether Ca2 + , alone , is able to shift muscle from the relaxed to the fully active state or whether cross-bridge binding also contributes to turning on muscle contraction .
	manualset3
214264	7	419637	7	NULL	NULL	0	NULL	turning on 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the field of muscle regulation , there is still controversy as to whether Ca2 + , alone , is able to shift muscle from the relaxed to the fully active state or whether cross-bridge binding also contributes to turning on muscle contraction .
	manualset3
214265	8	419637	7	NULL	NULL	0	NULL	muscle contraction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the field of muscle regulation , there is still controversy as to whether Ca2 + , alone , is able to shift muscle from the relaxed to the fully active state or whether cross-bridge binding also contributes to turning on muscle contraction .
	manualset3
214266	1	419638	7	NULL	NULL	0	NULL	Extinction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Extinction was associated with liver inflammation on tissue sections and appearance of antibodies against the transgene product , while vector genomes became undetectable in liver tissue by PCR .
	manualset3
214267	2	419638	7	NULL	NULL	0	NULL	liver inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Extinction was associated with liver inflammation on tissue sections and appearance of antibodies against the transgene product , while vector genomes became undetectable in liver tissue by PCR .
	manualset3
214268	3	419638	7	NULL	NULL	0	NULL	tissue sections	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Extinction was associated with liver inflammation on tissue sections and appearance of antibodies against the transgene product , while vector genomes became undetectable in liver tissue by PCR .
	manualset3
214269	4	419638	7	NULL	NULL	0	NULL	appearance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Extinction was associated with liver inflammation on tissue sections and appearance of antibodies against the transgene product , while vector genomes became undetectable in liver tissue by PCR .
	manualset3
214270	5	419638	7	NULL	NULL	0	NULL	antibodies 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Extinction was associated with liver inflammation on tissue sections and appearance of antibodies against the transgene product , while vector genomes became undetectable in liver tissue by PCR .
	manualset3
214271	6	419638	7	NULL	NULL	0	NULL	transgene product	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Extinction was associated with liver inflammation on tissue sections and appearance of antibodies against the transgene product , while vector genomes became undetectable in liver tissue by PCR .
	manualset3
214272	7	419638	7	NULL	NULL	0	NULL	vector genomes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Extinction was associated with liver inflammation on tissue sections and appearance of antibodies against the transgene product , while vector genomes became undetectable in liver tissue by PCR .
	manualset3
214273	8	419638	7	NULL	NULL	0	NULL	liver tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Extinction was associated with liver inflammation on tissue sections and appearance of antibodies against the transgene product , while vector genomes became undetectable in liver tissue by PCR .
	manualset3
214274	9	419638	7	NULL	NULL	0	NULL	PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Extinction was associated with liver inflammation on tissue sections and appearance of antibodies against the transgene product , while vector genomes became undetectable in liver tissue by PCR .
	manualset3
214275	1	419639	7	NULL	NULL	0	NULL	new strategy	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we develop a new strategy to manipulate 5-HT ( 1A ) autoreceptors in raphe nuclei without affecting 5-HT ( 1A ) heteroreceptors , generating mice with higher ( 1A-High ) or lower ( 1A-Low ) autoreceptor levels .
	manualset3
214276	2	419639	7	NULL	NULL	0	NULL	5-HT ( 1A ) autoreceptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we develop a new strategy to manipulate 5-HT ( 1A ) autoreceptors in raphe nuclei without affecting 5-HT ( 1A ) heteroreceptors , generating mice with higher ( 1A-High ) or lower ( 1A-Low ) autoreceptor levels .
	manualset3
214277	3	419639	7	NULL	NULL	0	NULL	raphe nuclei 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we develop a new strategy to manipulate 5-HT ( 1A ) autoreceptors in raphe nuclei without affecting 5-HT ( 1A ) heteroreceptors , generating mice with higher ( 1A-High ) or lower ( 1A-Low ) autoreceptor levels .
	manualset3
214278	4	419639	7	NULL	NULL	0	NULL	5-HT ( 1A ) heteroreceptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we develop a new strategy to manipulate 5-HT ( 1A ) autoreceptors in raphe nuclei without affecting 5-HT ( 1A ) heteroreceptors , generating mice with higher ( 1A-High ) or lower ( 1A-Low ) autoreceptor levels .
	manualset3
214279	5	419639	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we develop a new strategy to manipulate 5-HT ( 1A ) autoreceptors in raphe nuclei without affecting 5-HT ( 1A ) heteroreceptors , generating mice with higher ( 1A-High ) or lower ( 1A-Low ) autoreceptor levels .
	manualset3
214280	6	419639	7	NULL	NULL	NULL	NULL	1A-High	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Here we develop a new strategy to manipulate 5-HT ( 1A ) autoreceptors in raphe nuclei without affecting 5-HT ( 1A ) heteroreceptors , generating mice with higher ( 1A-High ) or lower ( 1A-Low ) autoreceptor levels .
	manualset3
214281	7	419639	7	NULL	NULL	0	NULL	1A-Low	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we develop a new strategy to manipulate 5-HT ( 1A ) autoreceptors in raphe nuclei without affecting 5-HT ( 1A ) heteroreceptors , generating mice with higher ( 1A-High ) or lower ( 1A-Low ) autoreceptor levels .
	manualset3
214282	8	419639	7	NULL	NULL	0	NULL	autoreceptor levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we develop a new strategy to manipulate 5-HT ( 1A ) autoreceptors in raphe nuclei without affecting 5-HT ( 1A ) heteroreceptors , generating mice with higher ( 1A-High ) or lower ( 1A-Low ) autoreceptor levels .
	manualset3
214283	1	419640	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A study was therefore undertaken and we report our findings of the first phase , in which Chinese people living with HIV/AIDS in Hong Kong were asked to explain their perceptions of QOL so as to identify their construct of QOL using a qualitative approach .
	manualset3
214284	2	419640	7	NULL	NULL	0	NULL	 findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A study was therefore undertaken and we report our findings of the first phase , in which Chinese people living with HIV/AIDS in Hong Kong were asked to explain their perceptions of QOL so as to identify their construct of QOL using a qualitative approach .
	manualset3
214285	3	419640	7	NULL	NULL	0	NULL	first phase	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A study was therefore undertaken and we report our findings of the first phase , in which Chinese people living with HIV/AIDS in Hong Kong were asked to explain their perceptions of QOL so as to identify their construct of QOL using a qualitative approach .
	manualset3
214286	4	419640	7	NULL	NULL	0	NULL	Chinese people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A study was therefore undertaken and we report our findings of the first phase , in which Chinese people living with HIV/AIDS in Hong Kong were asked to explain their perceptions of QOL so as to identify their construct of QOL using a qualitative approach .
	manualset3
214287	5	419640	7	NULL	NULL	0	NULL	HIV/AIDS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A study was therefore undertaken and we report our findings of the first phase , in which Chinese people living with HIV/AIDS in Hong Kong were asked to explain their perceptions of QOL so as to identify their construct of QOL using a qualitative approach .
	manualset3
214288	6	419640	7	NULL	NULL	0	NULL	Hong Kong 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A study was therefore undertaken and we report our findings of the first phase , in which Chinese people living with HIV/AIDS in Hong Kong were asked to explain their perceptions of QOL so as to identify their construct of QOL using a qualitative approach .
	manualset3
214289	7	419640	7	NULL	NULL	0	NULL	perceptions	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A study was therefore undertaken and we report our findings of the first phase , in which Chinese people living with HIV/AIDS in Hong Kong were asked to explain their perceptions of QOL so as to identify their construct of QOL using a qualitative approach .
	manualset3
214290	8	419640	7	NULL	NULL	0	NULL	QOL 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A study was therefore undertaken and we report our findings of the first phase , in which Chinese people living with HIV/AIDS in Hong Kong were asked to explain their perceptions of QOL so as to identify their construct of QOL using a qualitative approach .
	manualset3
214291	9	419640	7	NULL	NULL	0	NULL	construct	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A study was therefore undertaken and we report our findings of the first phase , in which Chinese people living with HIV/AIDS in Hong Kong were asked to explain their perceptions of QOL so as to identify their construct of QOL using a qualitative approach .
	manualset3
214292	10	419640	7	NULL	NULL	0	NULL	QOL	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A study was therefore undertaken and we report our findings of the first phase , in which Chinese people living with HIV/AIDS in Hong Kong were asked to explain their perceptions of QOL so as to identify their construct of QOL using a qualitative approach .
	manualset3
214293	11	419640	7	NULL	NULL	0	NULL	qualitative approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A study was therefore undertaken and we report our findings of the first phase , in which Chinese people living with HIV/AIDS in Hong Kong were asked to explain their perceptions of QOL so as to identify their construct of QOL using a qualitative approach .
	manualset3
214294	1	419641	7	NULL	NULL	0	NULL	Effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of psyllium on glucose and serum lipid responses in men with type 2 diabetes and hypercholesterolemia .
	manualset3
214295	2	419641	7	NULL	NULL	0	NULL	 psyllium	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of psyllium on glucose and serum lipid responses in men with type 2 diabetes and hypercholesterolemia .
	manualset3
214296	3	419641	7	NULL	NULL	0	NULL	glucose 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of psyllium on glucose and serum lipid responses in men with type 2 diabetes and hypercholesterolemia .
	manualset3
214297	4	419641	7	NULL	NULL	0	NULL	serum lipid responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of psyllium on glucose and serum lipid responses in men with type 2 diabetes and hypercholesterolemia .
	manualset3
214298	5	419641	7	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of psyllium on glucose and serum lipid responses in men with type 2 diabetes and hypercholesterolemia .
	manualset3
214299	6	419641	7	NULL	NULL	0	NULL	type 2 diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of psyllium on glucose and serum lipid responses in men with type 2 diabetes and hypercholesterolemia .
	manualset3
214300	7	419641	7	NULL	NULL	NULL	NULL	hypercholesterolemia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effects of psyllium on glucose and serum lipid responses in men with type 2 diabetes and hypercholesterolemia .
	manualset3
214301	1	419642	7	NULL	NULL	0	NULL	Cytotoxicity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cytotoxicity in alcoholic liver injury ( author 's transl ) ) .
	manualset3
214302	2	419642	7	NULL	NULL	0	NULL	alcoholic liver injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cytotoxicity in alcoholic liver injury ( author 's transl ) ) .
	manualset3
214303	3	419642	7	NULL	NULL	0	NULL	author 's transl	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cytotoxicity in alcoholic liver injury ( author 's transl ) ) .
	manualset3
214304	1	419643	7	NULL	NULL	0	NULL	protective immune responses 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although protective immune responses were induced , multiple inoculations were required and the percentage of protected chickens was too low ( & lt ; 50 % ) for commercial application .
	manualset3
214305	2	419643	7	NULL	NULL	0	NULL	multiple inoculations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although protective immune responses were induced , multiple inoculations were required and the percentage of protected chickens was too low ( & lt ; 50 % ) for commercial application .
	manualset3
214306	3	419643	7	NULL	NULL	0	NULL	percentage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although protective immune responses were induced , multiple inoculations were required and the percentage of protected chickens was too low ( & lt ; 50 % ) for commercial application .
	manualset3
214307	4	419643	7	NULL	NULL	0	NULL	protected chickens 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although protective immune responses were induced , multiple inoculations were required and the percentage of protected chickens was too low ( & lt ; 50 % ) for commercial application .
	manualset3
214308	5	419643	7	NULL	NULL	0	NULL	& lt ; 50 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although protective immune responses were induced , multiple inoculations were required and the percentage of protected chickens was too low ( & lt ; 50 % ) for commercial application .
	manualset3
214309	6	419643	7	NULL	NULL	0	NULL	commercial application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although protective immune responses were induced , multiple inoculations were required and the percentage of protected chickens was too low ( & lt ; 50 % ) for commercial application .
	manualset3
214310	1	419644	7	NULL	NULL	0	NULL	Modification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Modification of experimental Porphyromonas gingivalis murine infection by immunization with a polysaccharide-protein conjugate .
	manualset3
214311	2	419644	7	NULL	NULL	0	NULL	experimental Porphyromonas gingivalis murine infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Modification of experimental Porphyromonas gingivalis murine infection by immunization with a polysaccharide-protein conjugate .
	manualset3
214312	3	419644	7	NULL	NULL	0	NULL	immunization 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Modification of experimental Porphyromonas gingivalis murine infection by immunization with a polysaccharide-protein conjugate .
	manualset3
214313	4	419644	7	NULL	NULL	0	NULL	polysaccharide-protein conjugate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Modification of experimental Porphyromonas gingivalis murine infection by immunization with a polysaccharide-protein conjugate .
	manualset3
214314	1	419645	7	NULL	NULL	0	NULL	Antibiotic prophylaxis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic prophylaxis for bacterial meningitis : overuse and uncertain efficacy .
	manualset3
214315	2	419645	7	NULL	NULL	0	NULL	bacterial meningitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic prophylaxis for bacterial meningitis : overuse and uncertain efficacy .
	manualset3
214316	3	419645	7	NULL	NULL	0	NULL	 overuse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic prophylaxis for bacterial meningitis : overuse and uncertain efficacy .
	manualset3
214317	4	419645	7	NULL	NULL	0	NULL	 uncertain efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic prophylaxis for bacterial meningitis : overuse and uncertain efficacy .
	manualset3
215479	1	419646	7	NULL	NULL	0	NULL	Prevention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of dengue Fever : an exploratory school-community intervention involving students empowered as change agents ( * ) .
	manualset3
215480	2	419646	7	NULL	NULL	0	NULL	dengue Fever	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of dengue Fever : an exploratory school-community intervention involving students empowered as change agents ( * ) .
	manualset3
215481	3	419646	7	NULL	NULL	0	NULL	exploratory school-community intervention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of dengue Fever : an exploratory school-community intervention involving students empowered as change agents ( * ) .
	manualset3
215482	4	419646	7	NULL	NULL	0	NULL	students	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of dengue Fever : an exploratory school-community intervention involving students empowered as change agents ( * ) .
	manualset3
215483	5	419646	7	NULL	NULL	0	NULL	change agents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of dengue Fever : an exploratory school-community intervention involving students empowered as change agents ( * ) .
	manualset3
214318	1	419647	7	NULL	NULL	NULL	NULL	125I-Triton WR-1339 - loaded livers	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	However in the 125I-Triton WR-1339 - loaded livers cytochalasin B had no effect on the release of lysosomal enzymes or detergent , but reduced the loss of lactate dehydrogenase by about 50 % .
	manualset3
214319	2	419647	7	NULL	NULL	0	NULL	cytochalasin B 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However in the 125I-Triton WR-1339 - loaded livers cytochalasin B had no effect on the release of lysosomal enzymes or detergent , but reduced the loss of lactate dehydrogenase by about 50 % .
	manualset3
214320	3	419647	7	NULL	NULL	0	NULL	no effect 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However in the 125I-Triton WR-1339 - loaded livers cytochalasin B had no effect on the release of lysosomal enzymes or detergent , but reduced the loss of lactate dehydrogenase by about 50 % .
	manualset3
214321	4	419647	7	NULL	NULL	0	NULL	release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However in the 125I-Triton WR-1339 - loaded livers cytochalasin B had no effect on the release of lysosomal enzymes or detergent , but reduced the loss of lactate dehydrogenase by about 50 % .
	manualset3
214322	5	419647	7	NULL	NULL	0	NULL	lysosomal enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However in the 125I-Triton WR-1339 - loaded livers cytochalasin B had no effect on the release of lysosomal enzymes or detergent , but reduced the loss of lactate dehydrogenase by about 50 % .
	manualset3
214323	6	419647	7	NULL	NULL	0	NULL	detergent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However in the 125I-Triton WR-1339 - loaded livers cytochalasin B had no effect on the release of lysosomal enzymes or detergent , but reduced the loss of lactate dehydrogenase by about 50 % .
	manualset3
214324	7	419647	7	NULL	NULL	0	NULL	loss	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However in the 125I-Triton WR-1339 - loaded livers cytochalasin B had no effect on the release of lysosomal enzymes or detergent , but reduced the loss of lactate dehydrogenase by about 50 % .
	manualset3
214325	8	419647	7	NULL	NULL	0	NULL	lactate dehydrogenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However in the 125I-Triton WR-1339 - loaded livers cytochalasin B had no effect on the release of lysosomal enzymes or detergent , but reduced the loss of lactate dehydrogenase by about 50 % .
	manualset3
214326	9	419647	7	NULL	NULL	0	NULL	50 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However in the 125I-Triton WR-1339 - loaded livers cytochalasin B had no effect on the release of lysosomal enzymes or detergent , but reduced the loss of lactate dehydrogenase by about 50 % .
	manualset3
214327	1	419648	7	NULL	NULL	0	NULL	endogenous clock	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The endogenous clock is localized in the suprachiasmatic nucleus in mammals .
	manualset3
214328	2	419648	7	NULL	NULL	0	NULL	suprachiasmatic nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The endogenous clock is localized in the suprachiasmatic nucleus in mammals .
	manualset3
214329	3	419648	7	NULL	NULL	0	NULL	mammals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The endogenous clock is localized in the suprachiasmatic nucleus in mammals .
	manualset3
214330	1	419649	7	NULL	NULL	0	NULL	chapter	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This chapter takes a simple study on obesity and susceptibility to type 2 diabetes and uses it as an example that demonstrates how Partek GS can be used to analyze data arising from a microarray experiment .
	manualset3
214331	2	419649	7	NULL	NULL	0	NULL	simple study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This chapter takes a simple study on obesity and susceptibility to type 2 diabetes and uses it as an example that demonstrates how Partek GS can be used to analyze data arising from a microarray experiment .
	manualset3
214332	3	419649	7	NULL	NULL	0	NULL	obesity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This chapter takes a simple study on obesity and susceptibility to type 2 diabetes and uses it as an example that demonstrates how Partek GS can be used to analyze data arising from a microarray experiment .
	manualset3
214333	4	419649	7	NULL	NULL	0	NULL	susceptibility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This chapter takes a simple study on obesity and susceptibility to type 2 diabetes and uses it as an example that demonstrates how Partek GS can be used to analyze data arising from a microarray experiment .
	manualset3
214334	5	419649	7	NULL	NULL	0	NULL	type 2 diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This chapter takes a simple study on obesity and susceptibility to type 2 diabetes and uses it as an example that demonstrates how Partek GS can be used to analyze data arising from a microarray experiment .
	manualset3
214335	6	419649	7	NULL	NULL	0	NULL	example	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This chapter takes a simple study on obesity and susceptibility to type 2 diabetes and uses it as an example that demonstrates how Partek GS can be used to analyze data arising from a microarray experiment .
	manualset3
214336	7	419649	7	NULL	NULL	0	NULL	Partek GS	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This chapter takes a simple study on obesity and susceptibility to type 2 diabetes and uses it as an example that demonstrates how Partek GS can be used to analyze data arising from a microarray experiment .
	manualset3
214337	8	419649	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This chapter takes a simple study on obesity and susceptibility to type 2 diabetes and uses it as an example that demonstrates how Partek GS can be used to analyze data arising from a microarray experiment .
	manualset3
214338	9	419649	7	NULL	NULL	0	NULL	microarray experiment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This chapter takes a simple study on obesity and susceptibility to type 2 diabetes and uses it as an example that demonstrates how Partek GS can be used to analyze data arising from a microarray experiment .
	manualset3
214339	1	419650	7	NULL	NULL	0	NULL	Ultrasound	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound in speech therapy with adolescents and adults .
	manualset3
214340	2	419650	7	NULL	NULL	0	NULL	 speech therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound in speech therapy with adolescents and adults .
	manualset3
214341	3	419650	7	NULL	NULL	0	NULL	adolescents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound in speech therapy with adolescents and adults .
	manualset3
214342	4	419650	7	NULL	NULL	0	NULL	adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound in speech therapy with adolescents and adults .
	manualset3
214343	1	419651	7	NULL	NULL	0	NULL	oogonia	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the oogonia as well as in the leptotene and zygotene oocytes , the label is predominantly localized over chromosomes .
	manualset3
214344	2	419651	7	NULL	NULL	0	NULL	 leptotene oocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the oogonia as well as in the leptotene and zygotene oocytes , the label is predominantly localized over chromosomes .
	manualset3
214345	3	419651	7	NULL	NULL	0	NULL	 zygotene oocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the oogonia as well as in the leptotene and zygotene oocytes , the label is predominantly localized over chromosomes .
	manualset3
214346	4	419651	7	NULL	NULL	0	NULL	 label	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the oogonia as well as in the leptotene and zygotene oocytes , the label is predominantly localized over chromosomes .
	manualset3
214347	5	419651	7	NULL	NULL	0	NULL	chromosomes	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	In the oogonia as well as in the leptotene and zygotene oocytes , the label is predominantly localized over chromosomes .
	manualset3
214348	1	419652	7	NULL	NULL	0	NULL	Induction	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of abortion by intravenous and intra-uterine administration of prostaglandin F 2 .
	manualset3
214349	2	419652	7	NULL	NULL	0	NULL	abortion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of abortion by intravenous and intra-uterine administration of prostaglandin F 2 .
	manualset3
214350	3	419652	7	NULL	NULL	0	NULL	 intravenous administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of abortion by intravenous and intra-uterine administration of prostaglandin F 2 .
	manualset3
214351	4	419652	7	NULL	NULL	0	NULL	intra-uterine administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of abortion by intravenous and intra-uterine administration of prostaglandin F 2 .
	manualset3
214352	5	419652	7	NULL	NULL	0	NULL	prostaglandin F 2	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of abortion by intravenous and intra-uterine administration of prostaglandin F 2 .
	manualset3
214353	1	419653	7	NULL	NULL	0	NULL	Novel therapeutic strategies	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel therapeutic strategies , including a variety of antiangiogenic agents , are under investigation .
	manualset3
214354	2	419653	7	NULL	NULL	0	NULL	variety of antiangiogenic agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel therapeutic strategies , including a variety of antiangiogenic agents , are under investigation .
	manualset3
214355	3	419653	7	NULL	NULL	0	NULL	investigation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel therapeutic strategies , including a variety of antiangiogenic agents , are under investigation .
	manualset3
214356	1	419654	7	NULL	NULL	0	NULL	Intravenous anaesthesia	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous anaesthesia combined with peribulbar block in a child with suspected Duchenne muscular dystrophy .
	manualset3
214357	2	419654	7	NULL	NULL	0	NULL	peribulbar block	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous anaesthesia combined with peribulbar block in a child with suspected Duchenne muscular dystrophy .
	manualset3
214358	3	419654	7	NULL	NULL	0	NULL	child 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous anaesthesia combined with peribulbar block in a child with suspected Duchenne muscular dystrophy .
	manualset3
214359	4	419654	7	NULL	NULL	0	NULL	suspected Duchenne muscular dystrophy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous anaesthesia combined with peribulbar block in a child with suspected Duchenne muscular dystrophy .
	manualset3
214360	1	419655	7	NULL	NULL	0	NULL	Relations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relations between respiratory function and the radiological picture of asbestosis ) .
	manualset3
214361	2	419655	7	NULL	NULL	0	NULL	respiratory function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relations between respiratory function and the radiological picture of asbestosis ) .
	manualset3
214362	3	419655	7	NULL	NULL	0	NULL	radiological picture	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relations between respiratory function and the radiological picture of asbestosis ) .
	manualset3
214363	4	419655	7	NULL	NULL	0	NULL	asbestosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relations between respiratory function and the radiological picture of asbestosis ) .
	manualset3
214364	1	419656	7	NULL	NULL	0	NULL	 humans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in humans the mechanism of a functional progestin withdrawal is unclear , because progestin concentrations do not drop in maternal plasma preceding labor .
	manualset3
214365	2	419656	7	NULL	NULL	0	NULL	mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in humans the mechanism of a functional progestin withdrawal is unclear , because progestin concentrations do not drop in maternal plasma preceding labor .
	manualset3
214366	3	419656	7	NULL	NULL	0	NULL	functional progestin withdrawal	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in humans the mechanism of a functional progestin withdrawal is unclear , because progestin concentrations do not drop in maternal plasma preceding labor .
	manualset3
214367	4	419656	7	NULL	NULL	0	NULL	progestin concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in humans the mechanism of a functional progestin withdrawal is unclear , because progestin concentrations do not drop in maternal plasma preceding labor .
	manualset3
214368	5	419656	7	NULL	NULL	0	NULL	maternal plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in humans the mechanism of a functional progestin withdrawal is unclear , because progestin concentrations do not drop in maternal plasma preceding labor .
	manualset3
214369	6	419656	7	NULL	NULL	0	NULL	labor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , in humans the mechanism of a functional progestin withdrawal is unclear , because progestin concentrations do not drop in maternal plasma preceding labor .
	manualset3
214370	1	419657	7	NULL	NULL	0	NULL	 Staphylococcal strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The Staphylococcal strains , identified by `` The Simplified Lyogroups System '' were tested for their susceptibility to methicillin and some aminoglycosides .
	manualset3
214371	2	419657	7	NULL	NULL	0	NULL	`` The Simplified Lyogroups System '' 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The Staphylococcal strains , identified by `` The Simplified Lyogroups System '' were tested for their susceptibility to methicillin and some aminoglycosides .
	manualset3
214372	3	419657	7	NULL	NULL	0	NULL	susceptibility 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Staphylococcal strains , identified by `` The Simplified Lyogroups System '' were tested for their susceptibility to methicillin and some aminoglycosides .
	manualset3
214373	4	419657	7	NULL	NULL	0	NULL	methicillin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The Staphylococcal strains , identified by `` The Simplified Lyogroups System '' were tested for their susceptibility to methicillin and some aminoglycosides .
	manualset3
214374	5	419657	7	NULL	NULL	0	NULL	aminoglycosides	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The Staphylococcal strains , identified by `` The Simplified Lyogroups System '' were tested for their susceptibility to methicillin and some aminoglycosides .
	manualset3
214375	1	419658	7	NULL	NULL	0	NULL	zones	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , zones of anterograde and retrograde label in the thalamus were located with reference to architectonically defined subnuclei in the ventroposterior nucleus ( VP ) .
	manualset3
214376	2	419658	7	NULL	NULL	NULL	NULL	anterograde label	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Finally , zones of anterograde and retrograde label in the thalamus were located with reference to architectonically defined subnuclei in the ventroposterior nucleus ( VP ) .
	manualset3
214377	3	419658	7	NULL	NULL	NULL	NULL	retrograde label	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Finally , zones of anterograde and retrograde label in the thalamus were located with reference to architectonically defined subnuclei in the ventroposterior nucleus ( VP ) .
	manualset3
214378	4	419658	7	NULL	NULL	0	NULL	thalamus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , zones of anterograde and retrograde label in the thalamus were located with reference to architectonically defined subnuclei in the ventroposterior nucleus ( VP ) .
	manualset3
214379	5	419658	7	NULL	NULL	0	NULL	reference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , zones of anterograde and retrograde label in the thalamus were located with reference to architectonically defined subnuclei in the ventroposterior nucleus ( VP ) .
	manualset3
214380	6	419658	7	NULL	NULL	0	NULL	subnuclei	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , zones of anterograde and retrograde label in the thalamus were located with reference to architectonically defined subnuclei in the ventroposterior nucleus ( VP ) .
	manualset3
214381	7	419658	7	NULL	NULL	0	NULL	ventroposterior nucleus ( VP )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , zones of anterograde and retrograde label in the thalamus were located with reference to architectonically defined subnuclei in the ventroposterior nucleus ( VP ) .
	manualset3
214382	1	419659	7	NULL	NULL	0	NULL	hypothyroidism	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Although rare , hypothyroidism should be considered as a potential cause of rhabdomyolysis in pediatric patients undergoing a myopathy workup .
	manualset3
214383	2	419659	7	NULL	NULL	0	NULL	potential cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although rare , hypothyroidism should be considered as a potential cause of rhabdomyolysis in pediatric patients undergoing a myopathy workup .
	manualset3
214384	3	419659	7	NULL	NULL	0	NULL	rhabdomyolysis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Although rare , hypothyroidism should be considered as a potential cause of rhabdomyolysis in pediatric patients undergoing a myopathy workup .
	manualset3
214385	4	419659	7	NULL	NULL	0	NULL	pediatric patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although rare , hypothyroidism should be considered as a potential cause of rhabdomyolysis in pediatric patients undergoing a myopathy workup .
	manualset3
214386	5	419659	7	NULL	NULL	0	NULL	myopathy workup	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Although rare , hypothyroidism should be considered as a potential cause of rhabdomyolysis in pediatric patients undergoing a myopathy workup .
	manualset3
214387	1	419660	7	NULL	NULL	0	NULL	 interaction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	: its unique interaction with brown adipose tissue .
	manualset3
214388	2	419660	7	NULL	NULL	0	NULL	brown adipose tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	: its unique interaction with brown adipose tissue .
	manualset3
214389	1	419661	7	NULL	NULL	0	NULL	 initial leakage rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial leakage rate decreases rapidly with increasing pendant acyloxy chain length .
	manualset3
214390	2	419661	7	NULL	NULL	0	NULL	 pendant acyloxy chain length	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial leakage rate decreases rapidly with increasing pendant acyloxy chain length .
	manualset3
214391	1	419662	7	NULL	NULL	0	NULL	feeding	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiologically , feeding is a cycle of neurophysiologic activity , where sensory input travels to the CNS which sends motor signals out to the periphery .
	manualset3
214392	2	419662	7	NULL	NULL	0	NULL	cycle	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiologically , feeding is a cycle of neurophysiologic activity , where sensory input travels to the CNS which sends motor signals out to the periphery .
	manualset3
214393	3	419662	7	NULL	NULL	0	NULL	neurophysiologic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiologically , feeding is a cycle of neurophysiologic activity , where sensory input travels to the CNS which sends motor signals out to the periphery .
	manualset3
214394	4	419662	7	NULL	NULL	0	NULL	sensory input	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiologically , feeding is a cycle of neurophysiologic activity , where sensory input travels to the CNS which sends motor signals out to the periphery .
	manualset3
214395	5	419662	7	NULL	NULL	0	NULL	CNS	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiologically , feeding is a cycle of neurophysiologic activity , where sensory input travels to the CNS which sends motor signals out to the periphery .
	manualset3
214396	6	419662	7	NULL	NULL	0	NULL	motor signals 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiologically , feeding is a cycle of neurophysiologic activity , where sensory input travels to the CNS which sends motor signals out to the periphery .
	manualset3
214397	7	419662	7	NULL	NULL	0	NULL	periphery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Physiologically , feeding is a cycle of neurophysiologic activity , where sensory input travels to the CNS which sends motor signals out to the periphery .
	manualset3
214398	1	419663	7	NULL	NULL	0	NULL	Development	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Development of methods of local hyperthermia to achieve more marked tumor pathomorphism ) .
	manualset3
214399	2	419663	7	NULL	NULL	0	NULL	methods	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Development of methods of local hyperthermia to achieve more marked tumor pathomorphism ) .
	manualset3
214400	3	419663	7	NULL	NULL	0	NULL	local hyperthermia	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Development of methods of local hyperthermia to achieve more marked tumor pathomorphism ) .
	manualset3
214401	4	419663	7	NULL	NULL	0	NULL	tumor pathomorphism 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Development of methods of local hyperthermia to achieve more marked tumor pathomorphism ) .
	manualset3
214402	1	419664	7	NULL	NULL	0	NULL	crisis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Every crisis presents an opportunity , and today 's med-mal insurance squeeze is no exception .
	manualset3
214403	2	419664	7	NULL	NULL	NULL	NULL	opportunity	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Every crisis presents an opportunity , and today 's med-mal insurance squeeze is no exception .
	manualset3
214404	3	419664	7	NULL	NULL	0	NULL	today 's med-mal insurance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Every crisis presents an opportunity , and today 's med-mal insurance squeeze is no exception .
	manualset3
214405	4	419664	7	NULL	NULL	0	NULL	exception	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Every crisis presents an opportunity , and today 's med-mal insurance squeeze is no exception .
	manualset3
214406	1	419665	7	NULL	NULL	0	NULL	Ceramides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ceramides perturb the structure of phosphatidylcholine bilayers and modulate the activity of phospholipase A2 .
	manualset3
214407	2	419665	7	NULL	NULL	0	NULL	structure 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ceramides perturb the structure of phosphatidylcholine bilayers and modulate the activity of phospholipase A2 .
	manualset3
214408	3	419665	7	NULL	NULL	0	NULL	phosphatidylcholine bilayers	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ceramides perturb the structure of phosphatidylcholine bilayers and modulate the activity of phospholipase A2 .
	manualset3
214409	4	419665	7	NULL	NULL	0	NULL	activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ceramides perturb the structure of phosphatidylcholine bilayers and modulate the activity of phospholipase A2 .
	manualset3
214410	5	419665	7	NULL	NULL	0	NULL	phospholipase A2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Ceramides perturb the structure of phosphatidylcholine bilayers and modulate the activity of phospholipase A2 .
	manualset3
214411	1	419666	7	NULL	NULL	0	NULL	 dose dependent manner	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It occurred in a dose dependent manner with increasing serum concentration and was independent of previous blood transfusion or administered drugs .
	manualset3
214412	2	419666	7	NULL	NULL	0	NULL	serum concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It occurred in a dose dependent manner with increasing serum concentration and was independent of previous blood transfusion or administered drugs .
	manualset3
214413	3	419666	7	NULL	NULL	0	NULL	blood transfusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It occurred in a dose dependent manner with increasing serum concentration and was independent of previous blood transfusion or administered drugs .
	manualset3
214414	4	419666	7	NULL	NULL	0	NULL	drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	It occurred in a dose dependent manner with increasing serum concentration and was independent of previous blood transfusion or administered drugs .
	manualset3
214415	1	419667	7	NULL	NULL	NULL	NULL	professional circles	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although rarely discussed in professional circles , adult love is a powerful ideal that strongly influences both individual and relationship psychology .
	manualset3
214416	2	419667	7	NULL	NULL	0	NULL	adult love	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although rarely discussed in professional circles , adult love is a powerful ideal that strongly influences both individual and relationship psychology .
	manualset3
214417	3	419667	7	NULL	NULL	0	NULL	 individual 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Although rarely discussed in professional circles , adult love is a powerful ideal that strongly influences both individual and relationship psychology .
	manualset3
214418	4	419667	7	NULL	NULL	0	NULL	relationship psychology 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Although rarely discussed in professional circles , adult love is a powerful ideal that strongly influences both individual and relationship psychology .
	manualset3
214419	1	419668	7	NULL	NULL	0	NULL	regime	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We consider the regime when the cold plasma is not accelerated , requiring a/gammag & lt ; & lt ; 1 , where a is the laser parameter , proportional to the field amplitude , and gammag is the group-velocity Lorentz factor .
	manualset3
214420	2	419668	7	NULL	NULL	0	NULL	cold plasma	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We consider the regime when the cold plasma is not accelerated , requiring a/gammag & lt ; & lt ; 1 , where a is the laser parameter , proportional to the field amplitude , and gammag is the group-velocity Lorentz factor .
	manualset3
214421	3	419668	7	NULL	NULL	0	NULL	a/gammag & lt	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We consider the regime when the cold plasma is not accelerated , requiring a/gammag & lt ; & lt ; 1 , where a is the laser parameter , proportional to the field amplitude , and gammag is the group-velocity Lorentz factor .
	manualset3
214422	4	419668	7	NULL	NULL	0	NULL	& lt ; 1	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We consider the regime when the cold plasma is not accelerated , requiring a/gammag & lt ; & lt ; 1 , where a is the laser parameter , proportional to the field amplitude , and gammag is the group-velocity Lorentz factor .
	manualset3
214423	5	419668	7	NULL	NULL	NULL	NULL	 a	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We consider the regime when the cold plasma is not accelerated , requiring a/gammag & lt ; & lt ; 1 , where a is the laser parameter , proportional to the field amplitude , and gammag is the group-velocity Lorentz factor .
	manualset3
214424	6	419668	7	NULL	NULL	0	NULL	 laser parameter	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We consider the regime when the cold plasma is not accelerated , requiring a/gammag & lt ; & lt ; 1 , where a is the laser parameter , proportional to the field amplitude , and gammag is the group-velocity Lorentz factor .
	manualset3
214425	7	419668	7	NULL	NULL	0	NULL	field amplitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We consider the regime when the cold plasma is not accelerated , requiring a/gammag & lt ; & lt ; 1 , where a is the laser parameter , proportional to the field amplitude , and gammag is the group-velocity Lorentz factor .
	manualset3
214426	8	419668	7	NULL	NULL	0	NULL	gammag	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We consider the regime when the cold plasma is not accelerated , requiring a/gammag & lt ; & lt ; 1 , where a is the laser parameter , proportional to the field amplitude , and gammag is the group-velocity Lorentz factor .
	manualset3
214427	9	419668	7	NULL	NULL	0	NULL	group-velocity Lorentz factor	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We consider the regime when the cold plasma is not accelerated , requiring a/gammag & lt ; & lt ; 1 , where a is the laser parameter , proportional to the field amplitude , and gammag is the group-velocity Lorentz factor .
	manualset3
214428	1	419669	7	NULL	NULL	0	NULL	Thyrotropin-releasing hormone	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Thyrotropin-releasing hormone in specific nuclei of rat brain .
	manualset3
214429	2	419669	7	NULL	NULL	0	NULL	 nuclei	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Thyrotropin-releasing hormone in specific nuclei of rat brain .
	manualset3
214430	3	419669	7	NULL	NULL	0	NULL	rat brain 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Thyrotropin-releasing hormone in specific nuclei of rat brain .
	manualset3
214431	1	419670	7	NULL	NULL	0	NULL	Exposure 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Exposure of HeLa cells to TNF resulted in a rapid reduction in the number of TNF receptors without affecting the apparent binding affinity .
	manualset3
214432	2	419670	7	NULL	NULL	0	NULL	HeLa cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Exposure of HeLa cells to TNF resulted in a rapid reduction in the number of TNF receptors without affecting the apparent binding affinity .
	manualset3
214433	3	419670	7	NULL	NULL	0	NULL	 TNF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Exposure of HeLa cells to TNF resulted in a rapid reduction in the number of TNF receptors without affecting the apparent binding affinity .
	manualset3
214434	4	419670	7	NULL	NULL	0	NULL	rapid reduction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Exposure of HeLa cells to TNF resulted in a rapid reduction in the number of TNF receptors without affecting the apparent binding affinity .
	manualset3
214435	5	419670	7	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Exposure of HeLa cells to TNF resulted in a rapid reduction in the number of TNF receptors without affecting the apparent binding affinity .
	manualset3
214436	6	419670	7	NULL	NULL	0	NULL	TNF receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Exposure of HeLa cells to TNF resulted in a rapid reduction in the number of TNF receptors without affecting the apparent binding affinity .
	manualset3
214437	7	419670	7	NULL	NULL	0	NULL	binding affinity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Exposure of HeLa cells to TNF resulted in a rapid reduction in the number of TNF receptors without affecting the apparent binding affinity .
	manualset3
214438	1	419671	7	NULL	NULL	0	NULL	GRAIL	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrate that GRAIL is able to identify a subset of 16 deletions containing highly related genes ; many of these genes are expressed in the central nervous system and play a role in neuronal synapses .
	manualset3
214439	2	419671	7	NULL	NULL	0	NULL	subset 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrate that GRAIL is able to identify a subset of 16 deletions containing highly related genes ; many of these genes are expressed in the central nervous system and play a role in neuronal synapses .
	manualset3
214440	3	419671	7	NULL	NULL	NULL	NULL	 16 deletions	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We demonstrate that GRAIL is able to identify a subset of 16 deletions containing highly related genes ; many of these genes are expressed in the central nervous system and play a role in neuronal synapses .
	manualset3
214441	4	419671	7	NULL	NULL	0	NULL	highly related genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrate that GRAIL is able to identify a subset of 16 deletions containing highly related genes ; many of these genes are expressed in the central nervous system and play a role in neuronal synapses .
	manualset3
214442	5	419671	7	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrate that GRAIL is able to identify a subset of 16 deletions containing highly related genes ; many of these genes are expressed in the central nervous system and play a role in neuronal synapses .
	manualset3
214443	6	419671	7	NULL	NULL	0	NULL	central nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrate that GRAIL is able to identify a subset of 16 deletions containing highly related genes ; many of these genes are expressed in the central nervous system and play a role in neuronal synapses .
	manualset3
214444	7	419671	7	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrate that GRAIL is able to identify a subset of 16 deletions containing highly related genes ; many of these genes are expressed in the central nervous system and play a role in neuronal synapses .
	manualset3
214445	8	419671	7	NULL	NULL	NULL	NULL	neuronal synapses	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We demonstrate that GRAIL is able to identify a subset of 16 deletions containing highly related genes ; many of these genes are expressed in the central nervous system and play a role in neuronal synapses .
	manualset3
214446	1	419672	7	NULL	NULL	0	NULL	notable feature	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A notable feature of PMR1-mediated mRNA decay is that it acts on specific mRNAs while they are engaged by translating ribosomes .
	manualset3
214447	2	419672	7	NULL	NULL	0	NULL	PMR1-mediated mRNA decay	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A notable feature of PMR1-mediated mRNA decay is that it acts on specific mRNAs while they are engaged by translating ribosomes .
	manualset3
214448	3	419672	7	NULL	NULL	0	NULL	mRNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A notable feature of PMR1-mediated mRNA decay is that it acts on specific mRNAs while they are engaged by translating ribosomes .
	manualset3
214449	4	419672	7	NULL	NULL	0	NULL	 ribosomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A notable feature of PMR1-mediated mRNA decay is that it acts on specific mRNAs while they are engaged by translating ribosomes .
	manualset3
214450	1	419673	7	NULL	NULL	0	NULL	history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A history of childhood eczema was found to be more common among young persons , indicating an increase in the prevalence of atopic dermatitis .
	manualset3
214451	2	419673	7	NULL	NULL	0	NULL	childhood eczema	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A history of childhood eczema was found to be more common among young persons , indicating an increase in the prevalence of atopic dermatitis .
	manualset3
214452	3	419673	7	NULL	NULL	0	NULL	young persons	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A history of childhood eczema was found to be more common among young persons , indicating an increase in the prevalence of atopic dermatitis .
	manualset3
214453	4	419673	7	NULL	NULL	0	NULL	 increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A history of childhood eczema was found to be more common among young persons , indicating an increase in the prevalence of atopic dermatitis .
	manualset3
214454	5	419673	7	NULL	NULL	0	NULL	prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A history of childhood eczema was found to be more common among young persons , indicating an increase in the prevalence of atopic dermatitis .
	manualset3
214455	6	419673	7	NULL	NULL	0	NULL	atopic dermatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A history of childhood eczema was found to be more common among young persons , indicating an increase in the prevalence of atopic dermatitis .
	manualset3
214456	1	419674	7	NULL	NULL	0	NULL	synthetic peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	A synthetic peptide encompassing the binding site of the second zinc atom ( the ` structural ' zinc ) of alcohol dehydrogenase .
	manualset3
214457	2	419674	7	NULL	NULL	0	NULL	binding site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A synthetic peptide encompassing the binding site of the second zinc atom ( the ` structural ' zinc ) of alcohol dehydrogenase .
	manualset3
214458	3	419674	7	NULL	NULL	0	NULL	second zinc atom	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	A synthetic peptide encompassing the binding site of the second zinc atom ( the ` structural ' zinc ) of alcohol dehydrogenase .
	manualset3
214459	4	419674	7	NULL	NULL	0	NULL	` structural ' zinc	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A synthetic peptide encompassing the binding site of the second zinc atom ( the ` structural ' zinc ) of alcohol dehydrogenase .
	manualset3
214460	5	419674	7	NULL	NULL	0	NULL	alcohol dehydrogenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A synthetic peptide encompassing the binding site of the second zinc atom ( the ` structural ' zinc ) of alcohol dehydrogenase .
	manualset3
214461	1	419675	7	NULL	NULL	0	NULL	recent data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	We review recent data concerning the composition of breast milk and its adequacy to support infant growth in the first six months of life , as well as trials that support breastfeeding as an important method to delay or reduce the incidence of atopic diseases such as eczema , allergies , and asthma .
	manualset3
214462	2	419675	7	NULL	NULL	0	NULL	composition	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We review recent data concerning the composition of breast milk and its adequacy to support infant growth in the first six months of life , as well as trials that support breastfeeding as an important method to delay or reduce the incidence of atopic diseases such as eczema , allergies , and asthma .
	manualset3
214463	3	419675	7	NULL	NULL	0	NULL	 breast milk	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	We review recent data concerning the composition of breast milk and its adequacy to support infant growth in the first six months of life , as well as trials that support breastfeeding as an important method to delay or reduce the incidence of atopic diseases such as eczema , allergies , and asthma .
	manualset3
214464	4	419675	7	NULL	NULL	0	NULL	infant growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We review recent data concerning the composition of breast milk and its adequacy to support infant growth in the first six months of life , as well as trials that support breastfeeding as an important method to delay or reduce the incidence of atopic diseases such as eczema , allergies , and asthma .
	manualset3
214465	5	419675	7	NULL	NULL	0	NULL	first six months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	We review recent data concerning the composition of breast milk and its adequacy to support infant growth in the first six months of life , as well as trials that support breastfeeding as an important method to delay or reduce the incidence of atopic diseases such as eczema , allergies , and asthma .
	manualset3
214466	6	419675	7	NULL	NULL	0	NULL	 life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We review recent data concerning the composition of breast milk and its adequacy to support infant growth in the first six months of life , as well as trials that support breastfeeding as an important method to delay or reduce the incidence of atopic diseases such as eczema , allergies , and asthma .
	manualset3
214467	7	419675	7	NULL	NULL	0	NULL	trials	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We review recent data concerning the composition of breast milk and its adequacy to support infant growth in the first six months of life , as well as trials that support breastfeeding as an important method to delay or reduce the incidence of atopic diseases such as eczema , allergies , and asthma .
	manualset3
214468	8	419675	7	NULL	NULL	0	NULL	breastfeeding	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We review recent data concerning the composition of breast milk and its adequacy to support infant growth in the first six months of life , as well as trials that support breastfeeding as an important method to delay or reduce the incidence of atopic diseases such as eczema , allergies , and asthma .
	manualset3
214469	9	419675	7	NULL	NULL	0	NULL	method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We review recent data concerning the composition of breast milk and its adequacy to support infant growth in the first six months of life , as well as trials that support breastfeeding as an important method to delay or reduce the incidence of atopic diseases such as eczema , allergies , and asthma .
	manualset3
214470	10	419675	7	NULL	NULL	0	NULL	incidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We review recent data concerning the composition of breast milk and its adequacy to support infant growth in the first six months of life , as well as trials that support breastfeeding as an important method to delay or reduce the incidence of atopic diseases such as eczema , allergies , and asthma .
	manualset3
214471	11	419675	7	NULL	NULL	0	NULL	atopic diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We review recent data concerning the composition of breast milk and its adequacy to support infant growth in the first six months of life , as well as trials that support breastfeeding as an important method to delay or reduce the incidence of atopic diseases such as eczema , allergies , and asthma .
	manualset3
214472	12	419675	7	NULL	NULL	0	NULL	eczema	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We review recent data concerning the composition of breast milk and its adequacy to support infant growth in the first six months of life , as well as trials that support breastfeeding as an important method to delay or reduce the incidence of atopic diseases such as eczema , allergies , and asthma .
	manualset3
214473	13	419675	7	NULL	NULL	0	NULL	allergies	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We review recent data concerning the composition of breast milk and its adequacy to support infant growth in the first six months of life , as well as trials that support breastfeeding as an important method to delay or reduce the incidence of atopic diseases such as eczema , allergies , and asthma .
	manualset3
214474	14	419675	7	NULL	NULL	0	NULL	asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We review recent data concerning the composition of breast milk and its adequacy to support infant growth in the first six months of life , as well as trials that support breastfeeding as an important method to delay or reduce the incidence of atopic diseases such as eczema , allergies , and asthma .
	manualset3
214475	1	419676	7	NULL	NULL	0	NULL	 recent developments 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although recent developments in MS have enabled the identification and quantification of hundreds of phosphorylation sites from a given biological sample , phosphoproteome analysis by MS has been plagued by inconsistent reproducibility arising from automated selection of precursor ions for fragmentation , identification , and quantification .
	manualset3
214476	2	419676	7	NULL	NULL	0	NULL	MS	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although recent developments in MS have enabled the identification and quantification of hundreds of phosphorylation sites from a given biological sample , phosphoproteome analysis by MS has been plagued by inconsistent reproducibility arising from automated selection of precursor ions for fragmentation , identification , and quantification .
	manualset3
214477	3	419676	7	NULL	NULL	0	NULL	 identification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although recent developments in MS have enabled the identification and quantification of hundreds of phosphorylation sites from a given biological sample , phosphoproteome analysis by MS has been plagued by inconsistent reproducibility arising from automated selection of precursor ions for fragmentation , identification , and quantification .
	manualset3
214478	4	419676	7	NULL	NULL	0	NULL	quantification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although recent developments in MS have enabled the identification and quantification of hundreds of phosphorylation sites from a given biological sample , phosphoproteome analysis by MS has been plagued by inconsistent reproducibility arising from automated selection of precursor ions for fragmentation , identification , and quantification .
	manualset3
214479	5	419676	7	NULL	NULL	0	NULL	hundreds	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although recent developments in MS have enabled the identification and quantification of hundreds of phosphorylation sites from a given biological sample , phosphoproteome analysis by MS has been plagued by inconsistent reproducibility arising from automated selection of precursor ions for fragmentation , identification , and quantification .
	manualset3
214480	6	419676	7	NULL	NULL	0	NULL	phosphorylation sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although recent developments in MS have enabled the identification and quantification of hundreds of phosphorylation sites from a given biological sample , phosphoproteome analysis by MS has been plagued by inconsistent reproducibility arising from automated selection of precursor ions for fragmentation , identification , and quantification .
	manualset3
214481	7	419676	7	NULL	NULL	0	NULL	biological sample	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Although recent developments in MS have enabled the identification and quantification of hundreds of phosphorylation sites from a given biological sample , phosphoproteome analysis by MS has been plagued by inconsistent reproducibility arising from automated selection of precursor ions for fragmentation , identification , and quantification .
	manualset3
214482	8	419676	7	NULL	NULL	0	NULL	phosphoproteome analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although recent developments in MS have enabled the identification and quantification of hundreds of phosphorylation sites from a given biological sample , phosphoproteome analysis by MS has been plagued by inconsistent reproducibility arising from automated selection of precursor ions for fragmentation , identification , and quantification .
	manualset3
214483	9	419676	7	NULL	NULL	0	NULL	MS 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although recent developments in MS have enabled the identification and quantification of hundreds of phosphorylation sites from a given biological sample , phosphoproteome analysis by MS has been plagued by inconsistent reproducibility arising from automated selection of precursor ions for fragmentation , identification , and quantification .
	manualset3
214484	10	419676	7	NULL	NULL	0	NULL	 inconsistent reproducibility	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although recent developments in MS have enabled the identification and quantification of hundreds of phosphorylation sites from a given biological sample , phosphoproteome analysis by MS has been plagued by inconsistent reproducibility arising from automated selection of precursor ions for fragmentation , identification , and quantification .
	manualset3
214485	11	419676	7	NULL	NULL	0	NULL	automated selection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although recent developments in MS have enabled the identification and quantification of hundreds of phosphorylation sites from a given biological sample , phosphoproteome analysis by MS has been plagued by inconsistent reproducibility arising from automated selection of precursor ions for fragmentation , identification , and quantification .
	manualset3
214486	12	419676	7	NULL	NULL	0	NULL	precursor ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Although recent developments in MS have enabled the identification and quantification of hundreds of phosphorylation sites from a given biological sample , phosphoproteome analysis by MS has been plagued by inconsistent reproducibility arising from automated selection of precursor ions for fragmentation , identification , and quantification .
	manualset3
214487	13	419676	7	NULL	NULL	0	NULL	 fragmentation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although recent developments in MS have enabled the identification and quantification of hundreds of phosphorylation sites from a given biological sample , phosphoproteome analysis by MS has been plagued by inconsistent reproducibility arising from automated selection of precursor ions for fragmentation , identification , and quantification .
	manualset3
214488	14	419676	7	NULL	NULL	0	NULL	 identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although recent developments in MS have enabled the identification and quantification of hundreds of phosphorylation sites from a given biological sample , phosphoproteome analysis by MS has been plagued by inconsistent reproducibility arising from automated selection of precursor ions for fragmentation , identification , and quantification .
	manualset3
214489	15	419676	7	NULL	NULL	0	NULL	quantification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although recent developments in MS have enabled the identification and quantification of hundreds of phosphorylation sites from a given biological sample , phosphoproteome analysis by MS has been plagued by inconsistent reproducibility arising from automated selection of precursor ions for fragmentation , identification , and quantification .
	manualset3
214490	1	419677	7	NULL	NULL	0	NULL	 role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of neighboring acidic and basic residues is complex : for the majority of tyrosines that are nitrated the distance to the heteroatom of the closest charged side chain corresponds to the distance needed for suspected nitrating species to form hydrogen bond bridges between the tyrosine and that charged amino acid .
	manualset3
214491	2	419677	7	NULL	NULL	0	NULL	neighboring acidic residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of neighboring acidic and basic residues is complex : for the majority of tyrosines that are nitrated the distance to the heteroatom of the closest charged side chain corresponds to the distance needed for suspected nitrating species to form hydrogen bond bridges between the tyrosine and that charged amino acid .
	manualset3
214492	3	419677	7	NULL	NULL	0	NULL	basic residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of neighboring acidic and basic residues is complex : for the majority of tyrosines that are nitrated the distance to the heteroatom of the closest charged side chain corresponds to the distance needed for suspected nitrating species to form hydrogen bond bridges between the tyrosine and that charged amino acid .
	manualset3
214493	4	419677	7	NULL	NULL	0	NULL	tyrosines	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of neighboring acidic and basic residues is complex : for the majority of tyrosines that are nitrated the distance to the heteroatom of the closest charged side chain corresponds to the distance needed for suspected nitrating species to form hydrogen bond bridges between the tyrosine and that charged amino acid .
	manualset3
214494	5	419677	7	NULL	NULL	0	NULL	distance	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of neighboring acidic and basic residues is complex : for the majority of tyrosines that are nitrated the distance to the heteroatom of the closest charged side chain corresponds to the distance needed for suspected nitrating species to form hydrogen bond bridges between the tyrosine and that charged amino acid .
	manualset3
214495	6	419677	7	NULL	NULL	0	NULL	heteroatom 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of neighboring acidic and basic residues is complex : for the majority of tyrosines that are nitrated the distance to the heteroatom of the closest charged side chain corresponds to the distance needed for suspected nitrating species to form hydrogen bond bridges between the tyrosine and that charged amino acid .
	manualset3
214496	7	419677	7	NULL	NULL	0	NULL	closest charged side chain	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of neighboring acidic and basic residues is complex : for the majority of tyrosines that are nitrated the distance to the heteroatom of the closest charged side chain corresponds to the distance needed for suspected nitrating species to form hydrogen bond bridges between the tyrosine and that charged amino acid .
	manualset3
214497	8	419677	7	NULL	NULL	0	NULL	distance 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of neighboring acidic and basic residues is complex : for the majority of tyrosines that are nitrated the distance to the heteroatom of the closest charged side chain corresponds to the distance needed for suspected nitrating species to form hydrogen bond bridges between the tyrosine and that charged amino acid .
	manualset3
214498	9	419677	7	NULL	NULL	0	NULL	suspected nitrating species	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of neighboring acidic and basic residues is complex : for the majority of tyrosines that are nitrated the distance to the heteroatom of the closest charged side chain corresponds to the distance needed for suspected nitrating species to form hydrogen bond bridges between the tyrosine and that charged amino acid .
	manualset3
214499	10	419677	7	NULL	NULL	0	NULL	hydrogen bond bridges	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of neighboring acidic and basic residues is complex : for the majority of tyrosines that are nitrated the distance to the heteroatom of the closest charged side chain corresponds to the distance needed for suspected nitrating species to form hydrogen bond bridges between the tyrosine and that charged amino acid .
	manualset3
214500	11	419677	7	NULL	NULL	0	NULL	tyrosine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of neighboring acidic and basic residues is complex : for the majority of tyrosines that are nitrated the distance to the heteroatom of the closest charged side chain corresponds to the distance needed for suspected nitrating species to form hydrogen bond bridges between the tyrosine and that charged amino acid .
	manualset3
214501	12	419677	7	NULL	NULL	0	NULL	charged amino acid	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of neighboring acidic and basic residues is complex : for the majority of tyrosines that are nitrated the distance to the heteroatom of the closest charged side chain corresponds to the distance needed for suspected nitrating species to form hydrogen bond bridges between the tyrosine and that charged amino acid .
	manualset3
215484	13	419677	7	NULL	NULL	0	NULL	majority	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of neighboring acidic and basic residues is complex : for the majority of tyrosines that are nitrated the distance to the heteroatom of the closest charged side chain corresponds to the distance needed for suspected nitrating species to form hydrogen bond bridges between the tyrosine and that charged amino acid .
	manualset3
214502	1	419678	7	NULL	NULL	0	NULL	frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of food transfers decreased with increasing immature age , while the frequency of independent feeding and processing of food increased .
	manualset3
214503	2	419678	7	NULL	NULL	0	NULL	food transfers	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of food transfers decreased with increasing immature age , while the frequency of independent feeding and processing of food increased .
	manualset3
214504	3	419678	7	NULL	NULL	0	NULL	increasing immature age	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of food transfers decreased with increasing immature age , while the frequency of independent feeding and processing of food increased .
	manualset3
214505	4	419678	7	NULL	NULL	0	NULL	frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of food transfers decreased with increasing immature age , while the frequency of independent feeding and processing of food increased .
	manualset3
214506	5	419678	7	NULL	NULL	0	NULL	independent feeding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of food transfers decreased with increasing immature age , while the frequency of independent feeding and processing of food increased .
	manualset3
214507	6	419678	7	NULL	NULL	0	NULL	processing of food	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of food transfers decreased with increasing immature age , while the frequency of independent feeding and processing of food increased .
	manualset3
214508	1	419679	7	NULL	NULL	0	NULL	tinnitus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The tinnitus and vertigo are caused by random labyrinthine fluid movements , the headache and diplopia by reduced spinal fluid pressure .
	manualset3
214509	2	419679	7	NULL	NULL	0	NULL	vertigo	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The tinnitus and vertigo are caused by random labyrinthine fluid movements , the headache and diplopia by reduced spinal fluid pressure .
	manualset3
214510	3	419679	7	NULL	NULL	0	NULL	random labyrinthine fluid movements	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The tinnitus and vertigo are caused by random labyrinthine fluid movements , the headache and diplopia by reduced spinal fluid pressure .
	manualset3
214511	4	419679	7	NULL	NULL	0	NULL	headache	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The tinnitus and vertigo are caused by random labyrinthine fluid movements , the headache and diplopia by reduced spinal fluid pressure .
	manualset3
214512	5	419679	7	NULL	NULL	0	NULL	diplopia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The tinnitus and vertigo are caused by random labyrinthine fluid movements , the headache and diplopia by reduced spinal fluid pressure .
	manualset3
214513	6	419679	7	NULL	NULL	NULL	NULL	spinal fluid pressure	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The tinnitus and vertigo are caused by random labyrinthine fluid movements , the headache and diplopia by reduced spinal fluid pressure .
	manualset3
214514	1	419680	7	NULL	NULL	0	NULL	Neuronal cell bodies	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuronal cell bodies labeled with FB and/or PI were seen intermixed bilaterally through the entire rostrocaudal extent of the central caudal nucleus .
	manualset3
214515	2	419680	7	NULL	NULL	0	NULL	FB	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuronal cell bodies labeled with FB and/or PI were seen intermixed bilaterally through the entire rostrocaudal extent of the central caudal nucleus .
	manualset3
214516	3	419680	7	NULL	NULL	0	NULL	PI	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuronal cell bodies labeled with FB and/or PI were seen intermixed bilaterally through the entire rostrocaudal extent of the central caudal nucleus .
	manualset3
214517	4	419680	7	NULL	NULL	0	NULL	rostrocaudal extent 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuronal cell bodies labeled with FB and/or PI were seen intermixed bilaterally through the entire rostrocaudal extent of the central caudal nucleus .
	manualset3
214518	5	419680	7	NULL	NULL	0	NULL	central caudal nucleus 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuronal cell bodies labeled with FB and/or PI were seen intermixed bilaterally through the entire rostrocaudal extent of the central caudal nucleus .
	manualset3
214519	1	419681	7	NULL	NULL	0	NULL	level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Both the level of circulating immune complexes and that of complement are increased in these patients .
	manualset3
214520	2	419681	7	NULL	NULL	0	NULL	circulating immune complexes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Both the level of circulating immune complexes and that of complement are increased in these patients .
	manualset3
214521	3	419681	7	NULL	NULL	0	NULL	complement	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Both the level of circulating immune complexes and that of complement are increased in these patients .
	manualset3
214522	4	419681	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Both the level of circulating immune complexes and that of complement are increased in these patients .
	manualset3
214523	1	419682	7	NULL	NULL	0	NULL	serum alkaline phosphatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although serum alkaline phosphatase and inorganic phosphorus levels elevated slightly in the 5.0 % group , activities of alanine aminotransferase and aspartate aminotransferase , and levels of serum urea nitrogen and creatinine were not changed significantly .
	manualset3
214524	2	419682	7	NULL	NULL	0	NULL	inorganic phosphorus levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although serum alkaline phosphatase and inorganic phosphorus levels elevated slightly in the 5.0 % group , activities of alanine aminotransferase and aspartate aminotransferase , and levels of serum urea nitrogen and creatinine were not changed significantly .
	manualset3
214525	3	419682	7	NULL	NULL	0	NULL	5.0 % group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although serum alkaline phosphatase and inorganic phosphorus levels elevated slightly in the 5.0 % group , activities of alanine aminotransferase and aspartate aminotransferase , and levels of serum urea nitrogen and creatinine were not changed significantly .
	manualset3
214526	4	419682	7	NULL	NULL	0	NULL	activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although serum alkaline phosphatase and inorganic phosphorus levels elevated slightly in the 5.0 % group , activities of alanine aminotransferase and aspartate aminotransferase , and levels of serum urea nitrogen and creatinine were not changed significantly .
	manualset3
214527	5	419682	7	NULL	NULL	0	NULL	alanine aminotransferase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although serum alkaline phosphatase and inorganic phosphorus levels elevated slightly in the 5.0 % group , activities of alanine aminotransferase and aspartate aminotransferase , and levels of serum urea nitrogen and creatinine were not changed significantly .
	manualset3
214528	6	419682	7	NULL	NULL	0	NULL	aspartate aminotransferase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although serum alkaline phosphatase and inorganic phosphorus levels elevated slightly in the 5.0 % group , activities of alanine aminotransferase and aspartate aminotransferase , and levels of serum urea nitrogen and creatinine were not changed significantly .
	manualset3
214529	7	419682	7	NULL	NULL	0	NULL	levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although serum alkaline phosphatase and inorganic phosphorus levels elevated slightly in the 5.0 % group , activities of alanine aminotransferase and aspartate aminotransferase , and levels of serum urea nitrogen and creatinine were not changed significantly .
	manualset3
214530	8	419682	7	NULL	NULL	0	NULL	serum urea nitrogen	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although serum alkaline phosphatase and inorganic phosphorus levels elevated slightly in the 5.0 % group , activities of alanine aminotransferase and aspartate aminotransferase , and levels of serum urea nitrogen and creatinine were not changed significantly .
	manualset3
214531	9	419682	7	NULL	NULL	0	NULL	creatinine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although serum alkaline phosphatase and inorganic phosphorus levels elevated slightly in the 5.0 % group , activities of alanine aminotransferase and aspartate aminotransferase , and levels of serum urea nitrogen and creatinine were not changed significantly .
	manualset3
214532	1	419683	7	NULL	NULL	0	NULL	 plot 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A plot of ln ( D ) against ln ( p ( 0 ) / p ) , where D is the measured diffusion coefficient and p ( 0 ) and p are the partial water pressures at saturation and at a particular relative humidity , respectively , was observed to be linear in all cases ( i.e. , for differing lipids , lateral monolayer pressures , temperatures , and substrates ) , in accordance with the above-mentioned diffusion model .
	manualset3
214533	2	419683	7	NULL	NULL	0	NULL	ln ( D ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A plot of ln ( D ) against ln ( p ( 0 ) / p ) , where D is the measured diffusion coefficient and p ( 0 ) and p are the partial water pressures at saturation and at a particular relative humidity , respectively , was observed to be linear in all cases ( i.e. , for differing lipids , lateral monolayer pressures , temperatures , and substrates ) , in accordance with the above-mentioned diffusion model .
	manualset3
214534	3	419683	7	NULL	NULL	0	NULL	 ln ( p ( 0 ) / p )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A plot of ln ( D ) against ln ( p ( 0 ) / p ) , where D is the measured diffusion coefficient and p ( 0 ) and p are the partial water pressures at saturation and at a particular relative humidity , respectively , was observed to be linear in all cases ( i.e. , for differing lipids , lateral monolayer pressures , temperatures , and substrates ) , in accordance with the above-mentioned diffusion model .
	manualset3
214535	4	419683	7	NULL	NULL	0	NULL	D	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A plot of ln ( D ) against ln ( p ( 0 ) / p ) , where D is the measured diffusion coefficient and p ( 0 ) and p are the partial water pressures at saturation and at a particular relative humidity , respectively , was observed to be linear in all cases ( i.e. , for differing lipids , lateral monolayer pressures , temperatures , and substrates ) , in accordance with the above-mentioned diffusion model .
	manualset3
214536	5	419683	7	NULL	NULL	0	NULL	measured diffusion coefficient	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A plot of ln ( D ) against ln ( p ( 0 ) / p ) , where D is the measured diffusion coefficient and p ( 0 ) and p are the partial water pressures at saturation and at a particular relative humidity , respectively , was observed to be linear in all cases ( i.e. , for differing lipids , lateral monolayer pressures , temperatures , and substrates ) , in accordance with the above-mentioned diffusion model .
	manualset3
214537	6	419683	7	NULL	NULL	0	NULL	p ( 0 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A plot of ln ( D ) against ln ( p ( 0 ) / p ) , where D is the measured diffusion coefficient and p ( 0 ) and p are the partial water pressures at saturation and at a particular relative humidity , respectively , was observed to be linear in all cases ( i.e. , for differing lipids , lateral monolayer pressures , temperatures , and substrates ) , in accordance with the above-mentioned diffusion model .
	manualset3
214538	7	419683	7	NULL	NULL	0	NULL	 p	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A plot of ln ( D ) against ln ( p ( 0 ) / p ) , where D is the measured diffusion coefficient and p ( 0 ) and p are the partial water pressures at saturation and at a particular relative humidity , respectively , was observed to be linear in all cases ( i.e. , for differing lipids , lateral monolayer pressures , temperatures , and substrates ) , in accordance with the above-mentioned diffusion model .
	manualset3
214539	8	419683	7	NULL	NULL	0	NULL	partial water pressures	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A plot of ln ( D ) against ln ( p ( 0 ) / p ) , where D is the measured diffusion coefficient and p ( 0 ) and p are the partial water pressures at saturation and at a particular relative humidity , respectively , was observed to be linear in all cases ( i.e. , for differing lipids , lateral monolayer pressures , temperatures , and substrates ) , in accordance with the above-mentioned diffusion model .
	manualset3
214540	9	419683	7	NULL	NULL	0	NULL	saturation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A plot of ln ( D ) against ln ( p ( 0 ) / p ) , where D is the measured diffusion coefficient and p ( 0 ) and p are the partial water pressures at saturation and at a particular relative humidity , respectively , was observed to be linear in all cases ( i.e. , for differing lipids , lateral monolayer pressures , temperatures , and substrates ) , in accordance with the above-mentioned diffusion model .
	manualset3
214541	10	419683	7	NULL	NULL	0	NULL	relative humidity	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A plot of ln ( D ) against ln ( p ( 0 ) / p ) , where D is the measured diffusion coefficient and p ( 0 ) and p are the partial water pressures at saturation and at a particular relative humidity , respectively , was observed to be linear in all cases ( i.e. , for differing lipids , lateral monolayer pressures , temperatures , and substrates ) , in accordance with the above-mentioned diffusion model .
	manualset3
214542	11	419683	7	NULL	NULL	NULL	NULL	 linear	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A plot of ln ( D ) against ln ( p ( 0 ) / p ) , where D is the measured diffusion coefficient and p ( 0 ) and p are the partial water pressures at saturation and at a particular relative humidity , respectively , was observed to be linear in all cases ( i.e. , for differing lipids , lateral monolayer pressures , temperatures , and substrates ) , in accordance with the above-mentioned diffusion model .
	manualset3
214543	12	419683	7	NULL	NULL	0	NULL	 lipids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A plot of ln ( D ) against ln ( p ( 0 ) / p ) , where D is the measured diffusion coefficient and p ( 0 ) and p are the partial water pressures at saturation and at a particular relative humidity , respectively , was observed to be linear in all cases ( i.e. , for differing lipids , lateral monolayer pressures , temperatures , and substrates ) , in accordance with the above-mentioned diffusion model .
	manualset3
214544	13	419683	7	NULL	NULL	NULL	NULL	lateral monolayer pressures	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A plot of ln ( D ) against ln ( p ( 0 ) / p ) , where D is the measured diffusion coefficient and p ( 0 ) and p are the partial water pressures at saturation and at a particular relative humidity , respectively , was observed to be linear in all cases ( i.e. , for differing lipids , lateral monolayer pressures , temperatures , and substrates ) , in accordance with the above-mentioned diffusion model .
	manualset3
214545	14	419683	7	NULL	NULL	0	NULL	temperatures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A plot of ln ( D ) against ln ( p ( 0 ) / p ) , where D is the measured diffusion coefficient and p ( 0 ) and p are the partial water pressures at saturation and at a particular relative humidity , respectively , was observed to be linear in all cases ( i.e. , for differing lipids , lateral monolayer pressures , temperatures , and substrates ) , in accordance with the above-mentioned diffusion model .
	manualset3
214546	15	419683	7	NULL	NULL	0	NULL	substrates	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A plot of ln ( D ) against ln ( p ( 0 ) / p ) , where D is the measured diffusion coefficient and p ( 0 ) and p are the partial water pressures at saturation and at a particular relative humidity , respectively , was observed to be linear in all cases ( i.e. , for differing lipids , lateral monolayer pressures , temperatures , and substrates ) , in accordance with the above-mentioned diffusion model .
	manualset3
214547	16	419683	7	NULL	NULL	NULL	NULL	 diffusion model	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A plot of ln ( D ) against ln ( p ( 0 ) / p ) , where D is the measured diffusion coefficient and p ( 0 ) and p are the partial water pressures at saturation and at a particular relative humidity , respectively , was observed to be linear in all cases ( i.e. , for differing lipids , lateral monolayer pressures , temperatures , and substrates ) , in accordance with the above-mentioned diffusion model .
	manualset3
214548	1	419684	7	NULL	NULL	0	NULL	 influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of psychological factors on the self-management of insulin-dependent diabetes mellitus .
	manualset3
214549	2	419684	7	NULL	NULL	0	NULL	psychological factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of psychological factors on the self-management of insulin-dependent diabetes mellitus .
	manualset3
214550	3	419684	7	NULL	NULL	0	NULL	self-management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of psychological factors on the self-management of insulin-dependent diabetes mellitus .
	manualset3
214551	4	419684	7	NULL	NULL	0	NULL	insulin-dependent diabetes mellitus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of psychological factors on the self-management of insulin-dependent diabetes mellitus .
	manualset3
214552	1	419685	7	NULL	NULL	0	NULL	Data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Data were collected through semistructured interviews , observations , and chart reviews over three time periods ( before treatment , during treatment , and during rehabilitation ) over a period of 5 months .
	manualset3
214553	2	419685	7	NULL	NULL	0	NULL	semistructured interviews	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Data were collected through semistructured interviews , observations , and chart reviews over three time periods ( before treatment , during treatment , and during rehabilitation ) over a period of 5 months .
	manualset3
214554	3	419685	7	NULL	NULL	0	NULL	observations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Data were collected through semistructured interviews , observations , and chart reviews over three time periods ( before treatment , during treatment , and during rehabilitation ) over a period of 5 months .
	manualset3
214555	4	419685	7	NULL	NULL	0	NULL	chart reviews	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Data were collected through semistructured interviews , observations , and chart reviews over three time periods ( before treatment , during treatment , and during rehabilitation ) over a period of 5 months .
	manualset3
214556	5	419685	7	NULL	NULL	0	NULL	three time periods 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Data were collected through semistructured interviews , observations , and chart reviews over three time periods ( before treatment , during treatment , and during rehabilitation ) over a period of 5 months .
	manualset3
214557	6	419685	7	NULL	NULL	NULL	NULL	treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data were collected through semistructured interviews , observations , and chart reviews over three time periods ( before treatment , during treatment , and during rehabilitation ) over a period of 5 months .
	manualset3
214558	7	419685	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Data were collected through semistructured interviews , observations , and chart reviews over three time periods ( before treatment , during treatment , and during rehabilitation ) over a period of 5 months .
	manualset3
214559	8	419685	7	NULL	NULL	0	NULL	rehabilitation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Data were collected through semistructured interviews , observations , and chart reviews over three time periods ( before treatment , during treatment , and during rehabilitation ) over a period of 5 months .
	manualset3
214560	9	419685	7	NULL	NULL	NULL	NULL	period	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data were collected through semistructured interviews , observations , and chart reviews over three time periods ( before treatment , during treatment , and during rehabilitation ) over a period of 5 months .
	manualset3
214561	10	419685	7	NULL	NULL	0	NULL	5 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Data were collected through semistructured interviews , observations , and chart reviews over three time periods ( before treatment , during treatment , and during rehabilitation ) over a period of 5 months .
	manualset3
214562	1	419686	7	NULL	NULL	0	NULL	Myotoxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Myotoxicity was assessed by light and electronic microscopic analysis of extensor digitorum longus ( EDL ) muscles ; paralyzing activity was evaluated through the recording of both directly and indirectly evoked contractions of phrenic-diaphragm ( PD ) preparations .
	manualset3
214563	2	419686	7	NULL	NULL	0	NULL	 light microscopic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Myotoxicity was assessed by light and electronic microscopic analysis of extensor digitorum longus ( EDL ) muscles ; paralyzing activity was evaluated through the recording of both directly and indirectly evoked contractions of phrenic-diaphragm ( PD ) preparations .
	manualset3
214564	3	419686	7	NULL	NULL	0	NULL	electronic microscopic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Myotoxicity was assessed by light and electronic microscopic analysis of extensor digitorum longus ( EDL ) muscles ; paralyzing activity was evaluated through the recording of both directly and indirectly evoked contractions of phrenic-diaphragm ( PD ) preparations .
	manualset3
214565	4	419686	7	NULL	NULL	0	NULL	extensor digitorum longus ( EDL ) muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Myotoxicity was assessed by light and electronic microscopic analysis of extensor digitorum longus ( EDL ) muscles ; paralyzing activity was evaluated through the recording of both directly and indirectly evoked contractions of phrenic-diaphragm ( PD ) preparations .
	manualset3
214566	5	419686	7	NULL	NULL	0	NULL	paralyzing activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Myotoxicity was assessed by light and electronic microscopic analysis of extensor digitorum longus ( EDL ) muscles ; paralyzing activity was evaluated through the recording of both directly and indirectly evoked contractions of phrenic-diaphragm ( PD ) preparations .
	manualset3
214567	6	419686	7	NULL	NULL	0	NULL	recording	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Myotoxicity was assessed by light and electronic microscopic analysis of extensor digitorum longus ( EDL ) muscles ; paralyzing activity was evaluated through the recording of both directly and indirectly evoked contractions of phrenic-diaphragm ( PD ) preparations .
	manualset3
214568	7	419686	7	NULL	NULL	0	NULL	directly evoked contractions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Myotoxicity was assessed by light and electronic microscopic analysis of extensor digitorum longus ( EDL ) muscles ; paralyzing activity was evaluated through the recording of both directly and indirectly evoked contractions of phrenic-diaphragm ( PD ) preparations .
	manualset3
214569	8	419686	7	NULL	NULL	0	NULL	indirectly evoked contractions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Myotoxicity was assessed by light and electronic microscopic analysis of extensor digitorum longus ( EDL ) muscles ; paralyzing activity was evaluated through the recording of both directly and indirectly evoked contractions of phrenic-diaphragm ( PD ) preparations .
	manualset3
214570	9	419686	7	NULL	NULL	0	NULL	phrenic-diaphragm ( PD ) preparations 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Myotoxicity was assessed by light and electronic microscopic analysis of extensor digitorum longus ( EDL ) muscles ; paralyzing activity was evaluated through the recording of both directly and indirectly evoked contractions of phrenic-diaphragm ( PD ) preparations .
	manualset3
214571	1	419687	7	NULL	NULL	0	NULL	Parallel scanning	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel scanning of the foci enables us to observe real-time images of the specimen .
	manualset3
214572	2	419687	7	NULL	NULL	0	NULL	foci 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel scanning of the foci enables us to observe real-time images of the specimen .
	manualset3
214573	3	419687	7	NULL	NULL	0	NULL	real-time images	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel scanning of the foci enables us to observe real-time images of the specimen .
	manualset3
214574	4	419687	7	NULL	NULL	0	NULL	specimen	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Parallel scanning of the foci enables us to observe real-time images of the specimen .
	manualset3
214575	1	419688	7	NULL	NULL	0	NULL	Monoclonal antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibodies of two clones reacting with the nonnative forms of d-glyceraldehyde-3-phosphate dehydrogenase , EC 1.2.1.12 ( GAPDH ) , were obtained .
	manualset3
214576	2	419688	7	NULL	NULL	0	NULL	two clones	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibodies of two clones reacting with the nonnative forms of d-glyceraldehyde-3-phosphate dehydrogenase , EC 1.2.1.12 ( GAPDH ) , were obtained .
	manualset3
214577	3	419688	7	NULL	NULL	0	NULL	nonnative forms 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibodies of two clones reacting with the nonnative forms of d-glyceraldehyde-3-phosphate dehydrogenase , EC 1.2.1.12 ( GAPDH ) , were obtained .
	manualset3
214578	4	419688	7	NULL	NULL	0	NULL	d-glyceraldehyde-3-phosphate dehydrogenase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibodies of two clones reacting with the nonnative forms of d-glyceraldehyde-3-phosphate dehydrogenase , EC 1.2.1.12 ( GAPDH ) , were obtained .
	manualset3
214579	5	419688	7	NULL	NULL	0	NULL	EC 1.2.1.12	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibodies of two clones reacting with the nonnative forms of d-glyceraldehyde-3-phosphate dehydrogenase , EC 1.2.1.12 ( GAPDH ) , were obtained .
	manualset3
214580	6	419688	7	NULL	NULL	0	NULL	GAPDH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibodies of two clones reacting with the nonnative forms of d-glyceraldehyde-3-phosphate dehydrogenase , EC 1.2.1.12 ( GAPDH ) , were obtained .
	manualset3
214581	1	419689	7	NULL	NULL	0	NULL	response rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The response rate to second-line chemotherapy was 13 % ( 4/32 ) .
	manualset3
214582	2	419689	7	NULL	NULL	0	NULL	second-line chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The response rate to second-line chemotherapy was 13 % ( 4/32 ) .
	manualset3
214583	3	419689	7	NULL	NULL	0	NULL	13 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The response rate to second-line chemotherapy was 13 % ( 4/32 ) .
	manualset3
214584	4	419689	7	NULL	NULL	0	NULL	4/32	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The response rate to second-line chemotherapy was 13 % ( 4/32 ) .
	manualset3
214585	1	419690	7	NULL	NULL	0	NULL	Alcohol dehydrogenase 2 genotypes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Alcohol dehydrogenase 2 genotypes , maternal alcohol use , and infant outcome .
	manualset3
214586	2	419690	7	NULL	NULL	0	NULL	maternal alcohol use	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Alcohol dehydrogenase 2 genotypes , maternal alcohol use , and infant outcome .
	manualset3
214587	3	419690	7	NULL	NULL	0	NULL	infant outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Alcohol dehydrogenase 2 genotypes , maternal alcohol use , and infant outcome .
	manualset3
214588	1	419691	7	NULL	NULL	0	NULL	rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus in the rat , R ( aw ) is not simply a function of changes in lung volume .
	manualset3
214589	2	419691	7	NULL	NULL	0	NULL	R ( aw )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus in the rat , R ( aw ) is not simply a function of changes in lung volume .
	manualset3
214590	3	419691	7	NULL	NULL	NULL	NULL	function 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Thus in the rat , R ( aw ) is not simply a function of changes in lung volume .
	manualset3
214591	4	419691	7	NULL	NULL	0	NULL	lung volume	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus in the rat , R ( aw ) is not simply a function of changes in lung volume .
	manualset3
215485	5	419691	7	NULL	NULL	0	NULL	changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus in the rat , R ( aw ) is not simply a function of changes in lung volume .
	manualset3
214592	1	419692	7	NULL	NULL	0	NULL	 concept	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A concept of the dominance deviation was applied for the explanation of the epileptic seizure inheritance in the generations of P1 , F1 , F2 , B1 ( F1 X E1 mouse ) and B2 ( F1 X C57BL/6 mouse ) , in which initial rate increase of the seizure frequency , seizure-inducing rotation numbers and seizure formative period as a function of the population growth were undertaken to be phenotypic measures .
	manualset3
214593	2	419692	7	NULL	NULL	0	NULL	dominance deviation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A concept of the dominance deviation was applied for the explanation of the epileptic seizure inheritance in the generations of P1 , F1 , F2 , B1 ( F1 X E1 mouse ) and B2 ( F1 X C57BL/6 mouse ) , in which initial rate increase of the seizure frequency , seizure-inducing rotation numbers and seizure formative period as a function of the population growth were undertaken to be phenotypic measures .
	manualset3
214594	3	419692	7	NULL	NULL	0	NULL	explanation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A concept of the dominance deviation was applied for the explanation of the epileptic seizure inheritance in the generations of P1 , F1 , F2 , B1 ( F1 X E1 mouse ) and B2 ( F1 X C57BL/6 mouse ) , in which initial rate increase of the seizure frequency , seizure-inducing rotation numbers and seizure formative period as a function of the population growth were undertaken to be phenotypic measures .
	manualset3
214595	4	419692	7	NULL	NULL	NULL	NULL	epileptic seizure inheritance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A concept of the dominance deviation was applied for the explanation of the epileptic seizure inheritance in the generations of P1 , F1 , F2 , B1 ( F1 X E1 mouse ) and B2 ( F1 X C57BL/6 mouse ) , in which initial rate increase of the seizure frequency , seizure-inducing rotation numbers and seizure formative period as a function of the population growth were undertaken to be phenotypic measures .
	manualset3
214596	5	419692	7	NULL	NULL	0	NULL	 generations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A concept of the dominance deviation was applied for the explanation of the epileptic seizure inheritance in the generations of P1 , F1 , F2 , B1 ( F1 X E1 mouse ) and B2 ( F1 X C57BL/6 mouse ) , in which initial rate increase of the seizure frequency , seizure-inducing rotation numbers and seizure formative period as a function of the population growth were undertaken to be phenotypic measures .
	manualset3
214597	6	419692	7	NULL	NULL	0	NULL	 P1	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A concept of the dominance deviation was applied for the explanation of the epileptic seizure inheritance in the generations of P1 , F1 , F2 , B1 ( F1 X E1 mouse ) and B2 ( F1 X C57BL/6 mouse ) , in which initial rate increase of the seizure frequency , seizure-inducing rotation numbers and seizure formative period as a function of the population growth were undertaken to be phenotypic measures .
	manualset3
214598	7	419692	7	NULL	NULL	0	NULL	F1	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A concept of the dominance deviation was applied for the explanation of the epileptic seizure inheritance in the generations of P1 , F1 , F2 , B1 ( F1 X E1 mouse ) and B2 ( F1 X C57BL/6 mouse ) , in which initial rate increase of the seizure frequency , seizure-inducing rotation numbers and seizure formative period as a function of the population growth were undertaken to be phenotypic measures .
	manualset3
214599	8	419692	7	NULL	NULL	0	NULL	 F2	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A concept of the dominance deviation was applied for the explanation of the epileptic seizure inheritance in the generations of P1 , F1 , F2 , B1 ( F1 X E1 mouse ) and B2 ( F1 X C57BL/6 mouse ) , in which initial rate increase of the seizure frequency , seizure-inducing rotation numbers and seizure formative period as a function of the population growth were undertaken to be phenotypic measures .
	manualset3
214600	9	419692	7	NULL	NULL	0	NULL	B1 ( F1 X E1 mouse ) 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A concept of the dominance deviation was applied for the explanation of the epileptic seizure inheritance in the generations of P1 , F1 , F2 , B1 ( F1 X E1 mouse ) and B2 ( F1 X C57BL/6 mouse ) , in which initial rate increase of the seizure frequency , seizure-inducing rotation numbers and seizure formative period as a function of the population growth were undertaken to be phenotypic measures .
	manualset3
214601	10	419692	7	NULL	NULL	0	NULL	B2 ( F1 X C57BL/6 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A concept of the dominance deviation was applied for the explanation of the epileptic seizure inheritance in the generations of P1 , F1 , F2 , B1 ( F1 X E1 mouse ) and B2 ( F1 X C57BL/6 mouse ) , in which initial rate increase of the seizure frequency , seizure-inducing rotation numbers and seizure formative period as a function of the population growth were undertaken to be phenotypic measures .
	manualset3
214602	11	419692	7	NULL	NULL	0	NULL	mouse	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A concept of the dominance deviation was applied for the explanation of the epileptic seizure inheritance in the generations of P1 , F1 , F2 , B1 ( F1 X E1 mouse ) and B2 ( F1 X C57BL/6 mouse ) , in which initial rate increase of the seizure frequency , seizure-inducing rotation numbers and seizure formative period as a function of the population growth were undertaken to be phenotypic measures .
	manualset3
214603	12	419692	7	NULL	NULL	NULL	NULL	initial rate increase	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A concept of the dominance deviation was applied for the explanation of the epileptic seizure inheritance in the generations of P1 , F1 , F2 , B1 ( F1 X E1 mouse ) and B2 ( F1 X C57BL/6 mouse ) , in which initial rate increase of the seizure frequency , seizure-inducing rotation numbers and seizure formative period as a function of the population growth were undertaken to be phenotypic measures .
	manualset3
214604	13	419692	7	NULL	NULL	0	NULL	seizure frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A concept of the dominance deviation was applied for the explanation of the epileptic seizure inheritance in the generations of P1 , F1 , F2 , B1 ( F1 X E1 mouse ) and B2 ( F1 X C57BL/6 mouse ) , in which initial rate increase of the seizure frequency , seizure-inducing rotation numbers and seizure formative period as a function of the population growth were undertaken to be phenotypic measures .
	manualset3
214605	14	419692	7	NULL	NULL	0	NULL	seizure-inducing rotation numbers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A concept of the dominance deviation was applied for the explanation of the epileptic seizure inheritance in the generations of P1 , F1 , F2 , B1 ( F1 X E1 mouse ) and B2 ( F1 X C57BL/6 mouse ) , in which initial rate increase of the seizure frequency , seizure-inducing rotation numbers and seizure formative period as a function of the population growth were undertaken to be phenotypic measures .
	manualset3
214606	15	419692	7	NULL	NULL	0	NULL	seizure formative period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A concept of the dominance deviation was applied for the explanation of the epileptic seizure inheritance in the generations of P1 , F1 , F2 , B1 ( F1 X E1 mouse ) and B2 ( F1 X C57BL/6 mouse ) , in which initial rate increase of the seizure frequency , seizure-inducing rotation numbers and seizure formative period as a function of the population growth were undertaken to be phenotypic measures .
	manualset3
214607	16	419692	7	NULL	NULL	0	NULL	function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A concept of the dominance deviation was applied for the explanation of the epileptic seizure inheritance in the generations of P1 , F1 , F2 , B1 ( F1 X E1 mouse ) and B2 ( F1 X C57BL/6 mouse ) , in which initial rate increase of the seizure frequency , seizure-inducing rotation numbers and seizure formative period as a function of the population growth were undertaken to be phenotypic measures .
	manualset3
214608	17	419692	7	NULL	NULL	0	NULL	population growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A concept of the dominance deviation was applied for the explanation of the epileptic seizure inheritance in the generations of P1 , F1 , F2 , B1 ( F1 X E1 mouse ) and B2 ( F1 X C57BL/6 mouse ) , in which initial rate increase of the seizure frequency , seizure-inducing rotation numbers and seizure formative period as a function of the population growth were undertaken to be phenotypic measures .
	manualset3
214609	18	419692	7	NULL	NULL	0	NULL	phenotypic measures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A concept of the dominance deviation was applied for the explanation of the epileptic seizure inheritance in the generations of P1 , F1 , F2 , B1 ( F1 X E1 mouse ) and B2 ( F1 X C57BL/6 mouse ) , in which initial rate increase of the seizure frequency , seizure-inducing rotation numbers and seizure formative period as a function of the population growth were undertaken to be phenotypic measures .
	manualset3
214610	1	419693	7	NULL	NULL	0	NULL	Simple formulas	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Simple and useful formulas for frequency shifts and capacitance change versus biasing fields are obtained .
	manualset3
214611	2	419693	7	NULL	NULL	0	NULL	useful formulas	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Simple and useful formulas for frequency shifts and capacitance change versus biasing fields are obtained .
	manualset3
214612	3	419693	7	NULL	NULL	0	NULL	frequency shifts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Simple and useful formulas for frequency shifts and capacitance change versus biasing fields are obtained .
	manualset3
214613	4	419693	7	NULL	NULL	0	NULL	capacitance change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Simple and useful formulas for frequency shifts and capacitance change versus biasing fields are obtained .
	manualset3
214614	5	419693	7	NULL	NULL	0	NULL	biasing fields	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Simple and useful formulas for frequency shifts and capacitance change versus biasing fields are obtained .
	manualset3
214615	1	419694	7	NULL	NULL	0	NULL	14-kDa immunophilin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The 14-kDa immunophilin binds FK-506 and rapamycin whereas the 52-kDa immunophilin binds all three drugs .
	manualset3
214616	2	419694	7	NULL	NULL	0	NULL	FK-506	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The 14-kDa immunophilin binds FK-506 and rapamycin whereas the 52-kDa immunophilin binds all three drugs .
	manualset3
214617	3	419694	7	NULL	NULL	0	NULL	rapamycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The 14-kDa immunophilin binds FK-506 and rapamycin whereas the 52-kDa immunophilin binds all three drugs .
	manualset3
214618	4	419694	7	NULL	NULL	0	NULL	52-kDa immunophilin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The 14-kDa immunophilin binds FK-506 and rapamycin whereas the 52-kDa immunophilin binds all three drugs .
	manualset3
214619	5	419694	7	NULL	NULL	0	NULL	three drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The 14-kDa immunophilin binds FK-506 and rapamycin whereas the 52-kDa immunophilin binds all three drugs .
	manualset3
214620	1	419695	7	NULL	NULL	0	NULL	 suggestion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The suggestion that early exploratory operation be performed in all patients with stab wounds of the left lower chest in whom the diaphragm is likely to be injured is examined in detail .
	manualset3
214621	2	419695	7	NULL	NULL	0	NULL	early exploratory operation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The suggestion that early exploratory operation be performed in all patients with stab wounds of the left lower chest in whom the diaphragm is likely to be injured is examined in detail .
	manualset3
214622	3	419695	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The suggestion that early exploratory operation be performed in all patients with stab wounds of the left lower chest in whom the diaphragm is likely to be injured is examined in detail .
	manualset3
214623	4	419695	7	NULL	NULL	0	NULL	stab wounds	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The suggestion that early exploratory operation be performed in all patients with stab wounds of the left lower chest in whom the diaphragm is likely to be injured is examined in detail .
	manualset3
214624	5	419695	7	NULL	NULL	0	NULL	left lower chest	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The suggestion that early exploratory operation be performed in all patients with stab wounds of the left lower chest in whom the diaphragm is likely to be injured is examined in detail .
	manualset3
214625	6	419695	7	NULL	NULL	0	NULL	diaphragm	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The suggestion that early exploratory operation be performed in all patients with stab wounds of the left lower chest in whom the diaphragm is likely to be injured is examined in detail .
	manualset3
214626	1	419696	7	NULL	NULL	0	NULL	polyether impression materials	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The polyether impression materials exhibited the most consistent accuracy for a master cast to fabricate a complete-arch FPD .
	manualset3
214627	2	419696	7	NULL	NULL	0	NULL	 master cast	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The polyether impression materials exhibited the most consistent accuracy for a master cast to fabricate a complete-arch FPD .
	manualset3
214628	3	419696	7	NULL	NULL	0	NULL	complete-arch FPD	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The polyether impression materials exhibited the most consistent accuracy for a master cast to fabricate a complete-arch FPD .
	manualset3
214629	1	419697	7	NULL	NULL	0	NULL	material 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	This added material probably reflects the soluble proteins shifted into the nuclear matrix at high temperature .
	manualset3
214630	2	419697	7	NULL	NULL	0	NULL	soluble proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This added material probably reflects the soluble proteins shifted into the nuclear matrix at high temperature .
	manualset3
214631	3	419697	7	NULL	NULL	0	NULL	nuclear matrix 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	This added material probably reflects the soluble proteins shifted into the nuclear matrix at high temperature .
	manualset3
214632	4	419697	7	NULL	NULL	0	NULL	high temperature	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This added material probably reflects the soluble proteins shifted into the nuclear matrix at high temperature .
	manualset3
214633	1	419698	7	NULL	NULL	0	NULL	electron microscopic investigation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An electron microscopic investigation of the interaction in vitro of two major Z-line proteins , alpha-actinin and F-actin , indicated that the positions of alpha-actinin bridges between actin filaments are defined by relative azimuthal positions of actin subunits .
	manualset3
214634	2	419698	7	NULL	NULL	0	NULL	interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An electron microscopic investigation of the interaction in vitro of two major Z-line proteins , alpha-actinin and F-actin , indicated that the positions of alpha-actinin bridges between actin filaments are defined by relative azimuthal positions of actin subunits .
	manualset3
214635	3	419698	7	NULL	NULL	0	NULL	two major Z-line proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	An electron microscopic investigation of the interaction in vitro of two major Z-line proteins , alpha-actinin and F-actin , indicated that the positions of alpha-actinin bridges between actin filaments are defined by relative azimuthal positions of actin subunits .
	manualset3
214636	4	419698	7	NULL	NULL	0	NULL	alpha-actinin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	An electron microscopic investigation of the interaction in vitro of two major Z-line proteins , alpha-actinin and F-actin , indicated that the positions of alpha-actinin bridges between actin filaments are defined by relative azimuthal positions of actin subunits .
	manualset3
214637	5	419698	7	NULL	NULL	0	NULL	F-actin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	An electron microscopic investigation of the interaction in vitro of two major Z-line proteins , alpha-actinin and F-actin , indicated that the positions of alpha-actinin bridges between actin filaments are defined by relative azimuthal positions of actin subunits .
	manualset3
214638	6	419698	7	NULL	NULL	0	NULL	positions	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	An electron microscopic investigation of the interaction in vitro of two major Z-line proteins , alpha-actinin and F-actin , indicated that the positions of alpha-actinin bridges between actin filaments are defined by relative azimuthal positions of actin subunits .
	manualset3
214639	7	419698	7	NULL	NULL	0	NULL	alpha-actinin bridges	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	An electron microscopic investigation of the interaction in vitro of two major Z-line proteins , alpha-actinin and F-actin , indicated that the positions of alpha-actinin bridges between actin filaments are defined by relative azimuthal positions of actin subunits .
	manualset3
214640	8	419698	7	NULL	NULL	0	NULL	actin filaments	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	An electron microscopic investigation of the interaction in vitro of two major Z-line proteins , alpha-actinin and F-actin , indicated that the positions of alpha-actinin bridges between actin filaments are defined by relative azimuthal positions of actin subunits .
	manualset3
214641	9	419698	7	NULL	NULL	0	NULL	relative azimuthal positions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	An electron microscopic investigation of the interaction in vitro of two major Z-line proteins , alpha-actinin and F-actin , indicated that the positions of alpha-actinin bridges between actin filaments are defined by relative azimuthal positions of actin subunits .
	manualset3
214642	10	419698	7	NULL	NULL	0	NULL	actin subunits	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	An electron microscopic investigation of the interaction in vitro of two major Z-line proteins , alpha-actinin and F-actin , indicated that the positions of alpha-actinin bridges between actin filaments are defined by relative azimuthal positions of actin subunits .
	manualset3
214643	1	419699	7	NULL	NULL	0	NULL	hospital	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	He initially presented to hospital after six hours with mild hypotension and was treated with activated charcoal and intravenous fluids .
	manualset3
214644	2	419699	7	NULL	NULL	0	NULL	six hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	He initially presented to hospital after six hours with mild hypotension and was treated with activated charcoal and intravenous fluids .
	manualset3
214645	3	419699	7	NULL	NULL	0	NULL	mild hypotension 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	He initially presented to hospital after six hours with mild hypotension and was treated with activated charcoal and intravenous fluids .
	manualset3
214646	4	419699	7	NULL	NULL	0	NULL	activated charcoal 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	He initially presented to hospital after six hours with mild hypotension and was treated with activated charcoal and intravenous fluids .
	manualset3
214647	5	419699	7	NULL	NULL	0	NULL	 intravenous fluids	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	He initially presented to hospital after six hours with mild hypotension and was treated with activated charcoal and intravenous fluids .
	manualset3
214648	1	419700	7	NULL	NULL	0	NULL	several epidemiological studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although several epidemiological studies have investigated the association between antidepressants and the risk of developing cancer , different methodologies were applied and as a result most of the results were inconsistent .
	manualset3
214649	2	419700	7	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Although several epidemiological studies have investigated the association between antidepressants and the risk of developing cancer , different methodologies were applied and as a result most of the results were inconsistent .
	manualset3
214650	3	419700	7	NULL	NULL	0	NULL	antidepressants	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Although several epidemiological studies have investigated the association between antidepressants and the risk of developing cancer , different methodologies were applied and as a result most of the results were inconsistent .
	manualset3
214651	4	419700	7	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although several epidemiological studies have investigated the association between antidepressants and the risk of developing cancer , different methodologies were applied and as a result most of the results were inconsistent .
	manualset3
214652	5	419700	7	NULL	NULL	0	NULL	developing cancer	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although several epidemiological studies have investigated the association between antidepressants and the risk of developing cancer , different methodologies were applied and as a result most of the results were inconsistent .
	manualset3
214653	6	419700	7	NULL	NULL	0	NULL	different methodologies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although several epidemiological studies have investigated the association between antidepressants and the risk of developing cancer , different methodologies were applied and as a result most of the results were inconsistent .
	manualset3
214654	7	419700	7	NULL	NULL	0	NULL	 result 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although several epidemiological studies have investigated the association between antidepressants and the risk of developing cancer , different methodologies were applied and as a result most of the results were inconsistent .
	manualset3
214655	8	419700	7	NULL	NULL	0	NULL	 results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although several epidemiological studies have investigated the association between antidepressants and the risk of developing cancer , different methodologies were applied and as a result most of the results were inconsistent .
	manualset3
214656	1	419701	7	NULL	NULL	0	NULL	collateral circulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They were part of a collateral circulation that had developed from chronic obstruction of the inferior vena cava , where thrombosis had arisen in association with neonatal renal vein thrombosis .
	manualset3
214657	2	419701	7	NULL	NULL	0	NULL	chronic obstruction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They were part of a collateral circulation that had developed from chronic obstruction of the inferior vena cava , where thrombosis had arisen in association with neonatal renal vein thrombosis .
	manualset3
214658	3	419701	7	NULL	NULL	0	NULL	 inferior vena cava	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	They were part of a collateral circulation that had developed from chronic obstruction of the inferior vena cava , where thrombosis had arisen in association with neonatal renal vein thrombosis .
	manualset3
214659	4	419701	7	NULL	NULL	0	NULL	thrombosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	They were part of a collateral circulation that had developed from chronic obstruction of the inferior vena cava , where thrombosis had arisen in association with neonatal renal vein thrombosis .
	manualset3
214660	5	419701	7	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	They were part of a collateral circulation that had developed from chronic obstruction of the inferior vena cava , where thrombosis had arisen in association with neonatal renal vein thrombosis .
	manualset3
214661	6	419701	7	NULL	NULL	0	NULL	neonatal renal vein thrombosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	They were part of a collateral circulation that had developed from chronic obstruction of the inferior vena cava , where thrombosis had arisen in association with neonatal renal vein thrombosis .
	manualset3
214662	1	419702	7	NULL	NULL	0	NULL	behavioural assessment	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In behavioural assessment , treatment with ethanolic extract improved the cognitive function in the water maze and attenuated the elevated levels of AChE with increase in antioxidant enzymes , indicating the neuroprotection with increased levels of vitamin C. These findings suggest that ethanolic extract of P. viscida exerts anti-amnesiac effects and enhances cognitive function .
	manualset3
214663	2	419702	7	NULL	NULL	0	NULL	 treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In behavioural assessment , treatment with ethanolic extract improved the cognitive function in the water maze and attenuated the elevated levels of AChE with increase in antioxidant enzymes , indicating the neuroprotection with increased levels of vitamin C. These findings suggest that ethanolic extract of P. viscida exerts anti-amnesiac effects and enhances cognitive function .
	manualset3
214664	3	419702	7	NULL	NULL	0	NULL	ethanolic extract	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In behavioural assessment , treatment with ethanolic extract improved the cognitive function in the water maze and attenuated the elevated levels of AChE with increase in antioxidant enzymes , indicating the neuroprotection with increased levels of vitamin C. These findings suggest that ethanolic extract of P. viscida exerts anti-amnesiac effects and enhances cognitive function .
	manualset3
214665	4	419702	7	NULL	NULL	0	NULL	cognitive function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In behavioural assessment , treatment with ethanolic extract improved the cognitive function in the water maze and attenuated the elevated levels of AChE with increase in antioxidant enzymes , indicating the neuroprotection with increased levels of vitamin C. These findings suggest that ethanolic extract of P. viscida exerts anti-amnesiac effects and enhances cognitive function .
	manualset3
214666	5	419702	7	NULL	NULL	0	NULL	water maze	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In behavioural assessment , treatment with ethanolic extract improved the cognitive function in the water maze and attenuated the elevated levels of AChE with increase in antioxidant enzymes , indicating the neuroprotection with increased levels of vitamin C. These findings suggest that ethanolic extract of P. viscida exerts anti-amnesiac effects and enhances cognitive function .
	manualset3
214667	6	419702	7	NULL	NULL	0	NULL	elevated levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In behavioural assessment , treatment with ethanolic extract improved the cognitive function in the water maze and attenuated the elevated levels of AChE with increase in antioxidant enzymes , indicating the neuroprotection with increased levels of vitamin C. These findings suggest that ethanolic extract of P. viscida exerts anti-amnesiac effects and enhances cognitive function .
	manualset3
214668	7	419702	7	NULL	NULL	0	NULL	AChE	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In behavioural assessment , treatment with ethanolic extract improved the cognitive function in the water maze and attenuated the elevated levels of AChE with increase in antioxidant enzymes , indicating the neuroprotection with increased levels of vitamin C. These findings suggest that ethanolic extract of P. viscida exerts anti-amnesiac effects and enhances cognitive function .
	manualset3
214669	8	419702	7	NULL	NULL	0	NULL	antioxidant enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In behavioural assessment , treatment with ethanolic extract improved the cognitive function in the water maze and attenuated the elevated levels of AChE with increase in antioxidant enzymes , indicating the neuroprotection with increased levels of vitamin C. These findings suggest that ethanolic extract of P. viscida exerts anti-amnesiac effects and enhances cognitive function .
	manualset3
214670	9	419702	7	NULL	NULL	0	NULL	neuroprotection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In behavioural assessment , treatment with ethanolic extract improved the cognitive function in the water maze and attenuated the elevated levels of AChE with increase in antioxidant enzymes , indicating the neuroprotection with increased levels of vitamin C. These findings suggest that ethanolic extract of P. viscida exerts anti-amnesiac effects and enhances cognitive function .
	manualset3
214671	10	419702	7	NULL	NULL	0	NULL	 increased levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In behavioural assessment , treatment with ethanolic extract improved the cognitive function in the water maze and attenuated the elevated levels of AChE with increase in antioxidant enzymes , indicating the neuroprotection with increased levels of vitamin C. These findings suggest that ethanolic extract of P. viscida exerts anti-amnesiac effects and enhances cognitive function .
	manualset3
214672	11	419702	7	NULL	NULL	0	NULL	vitamin C	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In behavioural assessment , treatment with ethanolic extract improved the cognitive function in the water maze and attenuated the elevated levels of AChE with increase in antioxidant enzymes , indicating the neuroprotection with increased levels of vitamin C. These findings suggest that ethanolic extract of P. viscida exerts anti-amnesiac effects and enhances cognitive function .
	manualset3
214673	12	419702	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In behavioural assessment , treatment with ethanolic extract improved the cognitive function in the water maze and attenuated the elevated levels of AChE with increase in antioxidant enzymes , indicating the neuroprotection with increased levels of vitamin C. These findings suggest that ethanolic extract of P. viscida exerts anti-amnesiac effects and enhances cognitive function .
	manualset3
214674	13	419702	7	NULL	NULL	0	NULL	ethanolic extract	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In behavioural assessment , treatment with ethanolic extract improved the cognitive function in the water maze and attenuated the elevated levels of AChE with increase in antioxidant enzymes , indicating the neuroprotection with increased levels of vitamin C. These findings suggest that ethanolic extract of P. viscida exerts anti-amnesiac effects and enhances cognitive function .
	manualset3
214675	14	419702	7	NULL	NULL	0	NULL	 P. viscida	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In behavioural assessment , treatment with ethanolic extract improved the cognitive function in the water maze and attenuated the elevated levels of AChE with increase in antioxidant enzymes , indicating the neuroprotection with increased levels of vitamin C. These findings suggest that ethanolic extract of P. viscida exerts anti-amnesiac effects and enhances cognitive function .
	manualset3
214676	15	419702	7	NULL	NULL	0	NULL	anti-amnesiac effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In behavioural assessment , treatment with ethanolic extract improved the cognitive function in the water maze and attenuated the elevated levels of AChE with increase in antioxidant enzymes , indicating the neuroprotection with increased levels of vitamin C. These findings suggest that ethanolic extract of P. viscida exerts anti-amnesiac effects and enhances cognitive function .
	manualset3
214677	16	419702	7	NULL	NULL	0	NULL	cognitive function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In behavioural assessment , treatment with ethanolic extract improved the cognitive function in the water maze and attenuated the elevated levels of AChE with increase in antioxidant enzymes , indicating the neuroprotection with increased levels of vitamin C. These findings suggest that ethanolic extract of P. viscida exerts anti-amnesiac effects and enhances cognitive function .
	manualset3
214678	1	419703	7	NULL	NULL	0	NULL	Seasonal variation	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Seasonal variation in sudden-infant-death syndrome .
	manualset3
214679	2	419703	7	NULL	NULL	0	NULL	sudden-infant-death syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Seasonal variation in sudden-infant-death syndrome .
	manualset3
214680	1	419704	7	NULL	NULL	0	NULL	clinical approach	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A clinical approach to hypertension .
	manualset3
214681	2	419704	7	NULL	NULL	0	NULL	hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A clinical approach to hypertension .
	manualset3
214682	1	419705	7	NULL	NULL	0	NULL	Confirmation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Confirmation of these findings in further studies will be highly relevant in terms of road safety .
	manualset3
214683	2	419705	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Confirmation of these findings in further studies will be highly relevant in terms of road safety .
	manualset3
214684	3	419705	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Confirmation of these findings in further studies will be highly relevant in terms of road safety .
	manualset3
214685	4	419705	7	NULL	NULL	0	NULL	terms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Confirmation of these findings in further studies will be highly relevant in terms of road safety .
	manualset3
214686	5	419705	7	NULL	NULL	0	NULL	road safety	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Confirmation of these findings in further studies will be highly relevant in terms of road safety .
	manualset3
214687	1	419706	7	NULL	NULL	0	NULL	LAC9 protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The LAC9 protein is thought to bind to UAS and activate transcription of LAC4 ( L.V. Wray , M.M. Witte , R.C. Dickson , and M.I. Riley , Mol .
	manualset3
214688	2	419706	7	NULL	NULL	0	NULL	UAS	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The LAC9 protein is thought to bind to UAS and activate transcription of LAC4 ( L.V. Wray , M.M. Witte , R.C. Dickson , and M.I. Riley , Mol .
	manualset3
214689	3	419706	7	NULL	NULL	0	NULL	transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The LAC9 protein is thought to bind to UAS and activate transcription of LAC4 ( L.V. Wray , M.M. Witte , R.C. Dickson , and M.I. Riley , Mol .
	manualset3
214690	4	419706	7	NULL	NULL	0	NULL	LAC4	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The LAC9 protein is thought to bind to UAS and activate transcription of LAC4 ( L.V. Wray , M.M. Witte , R.C. Dickson , and M.I. Riley , Mol .
	manualset3
214691	5	419706	7	NULL	NULL	0	NULL	L.V. Wray , M.M. Witte , R.C. Dickson , and M.I. Riley , Mol .	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	The LAC9 protein is thought to bind to UAS and activate transcription of LAC4 ( L.V. Wray , M.M. Witte , R.C. Dickson , and M.I. Riley , Mol .
	manualset3
214692	1	419707	7	NULL	NULL	0	NULL	REF technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The REF technique has also proved valuable for our studies on meningococcal piliation and adherence .
	manualset3
214693	2	419707	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The REF technique has also proved valuable for our studies on meningococcal piliation and adherence .
	manualset3
214694	3	419707	7	NULL	NULL	0	NULL	meningococcal piliation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The REF technique has also proved valuable for our studies on meningococcal piliation and adherence .
	manualset3
214695	4	419707	7	NULL	NULL	0	NULL	adherence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The REF technique has also proved valuable for our studies on meningococcal piliation and adherence .
	manualset3
214696	1	419708	7	NULL	NULL	0	NULL	similar ratings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although similar ratings were given after melody and title cues , accuracy was better with title cues .
	manualset3
214697	2	419708	7	NULL	NULL	0	NULL	melody	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although similar ratings were given after melody and title cues , accuracy was better with title cues .
	manualset3
214698	3	419708	7	NULL	NULL	0	NULL	title cues	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although similar ratings were given after melody and title cues , accuracy was better with title cues .
	manualset3
214699	4	419708	7	NULL	NULL	0	NULL	 accuracy	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although similar ratings were given after melody and title cues , accuracy was better with title cues .
	manualset3
214700	5	419708	7	NULL	NULL	0	NULL	title cues	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although similar ratings were given after melody and title cues , accuracy was better with title cues .
	manualset3
214701	1	419709	7	NULL	NULL	0	NULL	Type A	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Type A : The synovial membrane is all around attached to the margin of the articular facet of the superior articular process of the sacrum .
	manualset3
214702	2	419709	7	NULL	NULL	0	NULL	synovial membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Type A : The synovial membrane is all around attached to the margin of the articular facet of the superior articular process of the sacrum .
	manualset3
214703	3	419709	7	NULL	NULL	NULL	NULL	margin of the articular facet 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Type A : The synovial membrane is all around attached to the margin of the articular facet of the superior articular process of the sacrum .
	manualset3
214704	4	419709	7	NULL	NULL	0	NULL	 superior articular process	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Type A : The synovial membrane is all around attached to the margin of the articular facet of the superior articular process of the sacrum .
	manualset3
214705	5	419709	7	NULL	NULL	0	NULL	sacrum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Type A : The synovial membrane is all around attached to the margin of the articular facet of the superior articular process of the sacrum .
	manualset3
214706	1	419710	7	NULL	NULL	0	NULL	novel binding site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel binding site for angiotensins II and III was recently discovered in brain membranes in the presence of the sulfhydryl reactive angiotensinase inhibitor parachloromercuribenzoate .
	manualset3
214707	2	419710	7	NULL	NULL	0	NULL	angiotensins II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel binding site for angiotensins II and III was recently discovered in brain membranes in the presence of the sulfhydryl reactive angiotensinase inhibitor parachloromercuribenzoate .
	manualset3
214708	3	419710	7	NULL	NULL	0	NULL	angiotensins III	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel binding site for angiotensins II and III was recently discovered in brain membranes in the presence of the sulfhydryl reactive angiotensinase inhibitor parachloromercuribenzoate .
	manualset3
214709	4	419710	7	NULL	NULL	0	NULL	brain membranes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel binding site for angiotensins II and III was recently discovered in brain membranes in the presence of the sulfhydryl reactive angiotensinase inhibitor parachloromercuribenzoate .
	manualset3
214710	5	419710	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel binding site for angiotensins II and III was recently discovered in brain membranes in the presence of the sulfhydryl reactive angiotensinase inhibitor parachloromercuribenzoate .
	manualset3
214711	6	419710	7	NULL	NULL	0	NULL	sulfhydryl reactive angiotensinase inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel binding site for angiotensins II and III was recently discovered in brain membranes in the presence of the sulfhydryl reactive angiotensinase inhibitor parachloromercuribenzoate .
	manualset3
214712	7	419710	7	NULL	NULL	0	NULL	parachloromercuribenzoate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel binding site for angiotensins II and III was recently discovered in brain membranes in the presence of the sulfhydryl reactive angiotensinase inhibitor parachloromercuribenzoate .
	manualset3
214713	1	419711	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , this study has shown that application of serotonin to these cells stimulates glycogenolysis and causes an increase in free cytosolic concentration of calcium that is not inhibited by the 5-HT2A selective antagonist , ketanserin .
	manualset3
214714	2	419711	7	NULL	NULL	0	NULL	application	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , this study has shown that application of serotonin to these cells stimulates glycogenolysis and causes an increase in free cytosolic concentration of calcium that is not inhibited by the 5-HT2A selective antagonist , ketanserin .
	manualset3
214715	3	419711	7	NULL	NULL	0	NULL	serotonin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , this study has shown that application of serotonin to these cells stimulates glycogenolysis and causes an increase in free cytosolic concentration of calcium that is not inhibited by the 5-HT2A selective antagonist , ketanserin .
	manualset3
214716	4	419711	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , this study has shown that application of serotonin to these cells stimulates glycogenolysis and causes an increase in free cytosolic concentration of calcium that is not inhibited by the 5-HT2A selective antagonist , ketanserin .
	manualset3
214717	5	419711	7	NULL	NULL	0	NULL	glycogenolysis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , this study has shown that application of serotonin to these cells stimulates glycogenolysis and causes an increase in free cytosolic concentration of calcium that is not inhibited by the 5-HT2A selective antagonist , ketanserin .
	manualset3
214718	6	419711	7	NULL	NULL	0	NULL	increase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , this study has shown that application of serotonin to these cells stimulates glycogenolysis and causes an increase in free cytosolic concentration of calcium that is not inhibited by the 5-HT2A selective antagonist , ketanserin .
	manualset3
214719	7	419711	7	NULL	NULL	0	NULL	free cytosolic concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , this study has shown that application of serotonin to these cells stimulates glycogenolysis and causes an increase in free cytosolic concentration of calcium that is not inhibited by the 5-HT2A selective antagonist , ketanserin .
	manualset3
214720	8	419711	7	NULL	NULL	0	NULL	calcium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , this study has shown that application of serotonin to these cells stimulates glycogenolysis and causes an increase in free cytosolic concentration of calcium that is not inhibited by the 5-HT2A selective antagonist , ketanserin .
	manualset3
214721	9	419711	7	NULL	NULL	0	NULL	5-HT2A selective antagonist	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , this study has shown that application of serotonin to these cells stimulates glycogenolysis and causes an increase in free cytosolic concentration of calcium that is not inhibited by the 5-HT2A selective antagonist , ketanserin .
	manualset3
214722	10	419711	7	NULL	NULL	0	NULL	ketanserin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , this study has shown that application of serotonin to these cells stimulates glycogenolysis and causes an increase in free cytosolic concentration of calcium that is not inhibited by the 5-HT2A selective antagonist , ketanserin .
	manualset3
214723	1	419712	7	NULL	NULL	0	NULL	repetitive-sequence-based PCR ( rep-PCR )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using repetitive-sequence-based PCR ( rep-PCR ) with 2 primer pairs ( ERIC and REP ) , pulsed-field gel electrophoresis and phage typing we found that the laboratory technician was infected with the same S. paratyphi B clone as the 14 tourists .
	manualset3
214724	2	419712	7	NULL	NULL	0	NULL	2 primer pairs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using repetitive-sequence-based PCR ( rep-PCR ) with 2 primer pairs ( ERIC and REP ) , pulsed-field gel electrophoresis and phage typing we found that the laboratory technician was infected with the same S. paratyphi B clone as the 14 tourists .
	manualset3
214725	3	419712	7	NULL	NULL	0	NULL	ERIC	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using repetitive-sequence-based PCR ( rep-PCR ) with 2 primer pairs ( ERIC and REP ) , pulsed-field gel electrophoresis and phage typing we found that the laboratory technician was infected with the same S. paratyphi B clone as the 14 tourists .
	manualset3
214726	4	419712	7	NULL	NULL	0	NULL	 REP 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using repetitive-sequence-based PCR ( rep-PCR ) with 2 primer pairs ( ERIC and REP ) , pulsed-field gel electrophoresis and phage typing we found that the laboratory technician was infected with the same S. paratyphi B clone as the 14 tourists .
	manualset3
214727	5	419712	7	NULL	NULL	0	NULL	pulsed-field gel electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using repetitive-sequence-based PCR ( rep-PCR ) with 2 primer pairs ( ERIC and REP ) , pulsed-field gel electrophoresis and phage typing we found that the laboratory technician was infected with the same S. paratyphi B clone as the 14 tourists .
	manualset3
214728	6	419712	7	NULL	NULL	0	NULL	phage typing 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using repetitive-sequence-based PCR ( rep-PCR ) with 2 primer pairs ( ERIC and REP ) , pulsed-field gel electrophoresis and phage typing we found that the laboratory technician was infected with the same S. paratyphi B clone as the 14 tourists .
	manualset3
214729	7	419712	7	NULL	NULL	0	NULL	laboratory technician	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Using repetitive-sequence-based PCR ( rep-PCR ) with 2 primer pairs ( ERIC and REP ) , pulsed-field gel electrophoresis and phage typing we found that the laboratory technician was infected with the same S. paratyphi B clone as the 14 tourists .
	manualset3
214730	8	419712	7	NULL	NULL	0	NULL	S. paratyphi B clone	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Using repetitive-sequence-based PCR ( rep-PCR ) with 2 primer pairs ( ERIC and REP ) , pulsed-field gel electrophoresis and phage typing we found that the laboratory technician was infected with the same S. paratyphi B clone as the 14 tourists .
	manualset3
214731	9	419712	7	NULL	NULL	0	NULL	14 tourists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using repetitive-sequence-based PCR ( rep-PCR ) with 2 primer pairs ( ERIC and REP ) , pulsed-field gel electrophoresis and phage typing we found that the laboratory technician was infected with the same S. paratyphi B clone as the 14 tourists .
	manualset3
214732	1	419713	7	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We also found that exposure of astrocytes to MA results in activation of NF-B through the phosphorylation of IB - , followed by translocation of active NF-B from the cytoplasm to the nucleus .
	manualset3
214733	2	419713	7	NULL	NULL	0	NULL	astrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We also found that exposure of astrocytes to MA results in activation of NF-B through the phosphorylation of IB - , followed by translocation of active NF-B from the cytoplasm to the nucleus .
	manualset3
214734	3	419713	7	NULL	NULL	0	NULL	MA	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	We also found that exposure of astrocytes to MA results in activation of NF-B through the phosphorylation of IB - , followed by translocation of active NF-B from the cytoplasm to the nucleus .
	manualset3
214735	4	419713	7	NULL	NULL	NULL	NULL	NF-B 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We also found that exposure of astrocytes to MA results in activation of NF-B through the phosphorylation of IB - , followed by translocation of active NF-B from the cytoplasm to the nucleus .
	manualset3
214736	5	419713	7	NULL	NULL	0	NULL	phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We also found that exposure of astrocytes to MA results in activation of NF-B through the phosphorylation of IB - , followed by translocation of active NF-B from the cytoplasm to the nucleus .
	manualset3
214737	6	419713	7	NULL	NULL	0	NULL	IB	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We also found that exposure of astrocytes to MA results in activation of NF-B through the phosphorylation of IB - , followed by translocation of active NF-B from the cytoplasm to the nucleus .
	manualset3
214738	7	419713	7	NULL	NULL	0	NULL	translocation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We also found that exposure of astrocytes to MA results in activation of NF-B through the phosphorylation of IB - , followed by translocation of active NF-B from the cytoplasm to the nucleus .
	manualset3
214739	8	419713	7	NULL	NULL	NULL	NULL	active NF-B	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We also found that exposure of astrocytes to MA results in activation of NF-B through the phosphorylation of IB - , followed by translocation of active NF-B from the cytoplasm to the nucleus .
	manualset3
214740	9	419713	7	NULL	NULL	0	NULL	cytoplasm	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	We also found that exposure of astrocytes to MA results in activation of NF-B through the phosphorylation of IB - , followed by translocation of active NF-B from the cytoplasm to the nucleus .
	manualset3
214741	10	419713	7	NULL	NULL	0	NULL	 nucleus 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	We also found that exposure of astrocytes to MA results in activation of NF-B through the phosphorylation of IB - , followed by translocation of active NF-B from the cytoplasm to the nucleus .
	manualset3
214742	1	419714	7	NULL	NULL	NULL	NULL	FIBRIN CLOTS	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	FIBRIN CLOTS , FIBRIN FILMS , AND FIBRINOGEN PLASTICS .
	manualset3
214743	2	419714	7	NULL	NULL	0	NULL	FIBRIN FILMS	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	FIBRIN CLOTS , FIBRIN FILMS , AND FIBRINOGEN PLASTICS .
	manualset3
214744	3	419714	7	NULL	NULL	0	NULL	FIBRINOGEN PLASTICS	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	FIBRIN CLOTS , FIBRIN FILMS , AND FIBRINOGEN PLASTICS .
	manualset3
214745	1	419715	7	NULL	NULL	0	NULL	R3	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with R3 , the - sheet structure and nanofibers formed by R4 are more stable ; they change to random coil and unordered aggregation at higher temperature .
	manualset3
214746	2	419715	7	NULL	NULL	0	NULL	sheet structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with R3 , the - sheet structure and nanofibers formed by R4 are more stable ; they change to random coil and unordered aggregation at higher temperature .
	manualset3
214747	3	419715	7	NULL	NULL	0	NULL	nanofibers	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with R3 , the - sheet structure and nanofibers formed by R4 are more stable ; they change to random coil and unordered aggregation at higher temperature .
	manualset3
214748	4	419715	7	NULL	NULL	0	NULL	R4 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with R3 , the - sheet structure and nanofibers formed by R4 are more stable ; they change to random coil and unordered aggregation at higher temperature .
	manualset3
214749	5	419715	7	NULL	NULL	0	NULL	random coil	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with R3 , the - sheet structure and nanofibers formed by R4 are more stable ; they change to random coil and unordered aggregation at higher temperature .
	manualset3
214750	6	419715	7	NULL	NULL	0	NULL	 unordered aggregation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with R3 , the - sheet structure and nanofibers formed by R4 are more stable ; they change to random coil and unordered aggregation at higher temperature .
	manualset3
214751	7	419715	7	NULL	NULL	0	NULL	higher temperature	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with R3 , the - sheet structure and nanofibers formed by R4 are more stable ; they change to random coil and unordered aggregation at higher temperature .
	manualset3
214752	1	419716	7	NULL	NULL	NULL	NULL	Silk sutures	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Silk sutures containing either FPB , fibrinopeptide A ( FPA ) , lipopolysaccharide ( LPS ) , or saline control were prepared .
	manualset3
214753	2	419716	7	NULL	NULL	0	NULL	FPB	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Silk sutures containing either FPB , fibrinopeptide A ( FPA ) , lipopolysaccharide ( LPS ) , or saline control were prepared .
	manualset3
214754	3	419716	7	NULL	NULL	0	NULL	fibrinopeptide A ( FPA )	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Silk sutures containing either FPB , fibrinopeptide A ( FPA ) , lipopolysaccharide ( LPS ) , or saline control were prepared .
	manualset3
214755	4	419716	7	NULL	NULL	0	NULL	lipopolysaccharide ( LPS )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Silk sutures containing either FPB , fibrinopeptide A ( FPA ) , lipopolysaccharide ( LPS ) , or saline control were prepared .
	manualset3
214756	5	419716	7	NULL	NULL	0	NULL	saline control 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Silk sutures containing either FPB , fibrinopeptide A ( FPA ) , lipopolysaccharide ( LPS ) , or saline control were prepared .
	manualset3
214757	1	419717	7	NULL	NULL	0	NULL	 social evolutionary theory	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although social evolutionary theory has mainly dealt with helping behaviors , competition for limited resources creates ecological conditions in which an actor may benefit from expressing behaviors that reduce the vital rates of neighbors .
	manualset3
214758	2	419717	7	NULL	NULL	NULL	NULL	 behaviors	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although social evolutionary theory has mainly dealt with helping behaviors , competition for limited resources creates ecological conditions in which an actor may benefit from expressing behaviors that reduce the vital rates of neighbors .
	manualset3
214759	3	419717	7	NULL	NULL	0	NULL	competition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although social evolutionary theory has mainly dealt with helping behaviors , competition for limited resources creates ecological conditions in which an actor may benefit from expressing behaviors that reduce the vital rates of neighbors .
	manualset3
214760	4	419717	7	NULL	NULL	0	NULL	limited resources	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although social evolutionary theory has mainly dealt with helping behaviors , competition for limited resources creates ecological conditions in which an actor may benefit from expressing behaviors that reduce the vital rates of neighbors .
	manualset3
214761	5	419717	7	NULL	NULL	0	NULL	ecological conditions	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Although social evolutionary theory has mainly dealt with helping behaviors , competition for limited resources creates ecological conditions in which an actor may benefit from expressing behaviors that reduce the vital rates of neighbors .
	manualset3
214762	6	419717	7	NULL	NULL	0	NULL	actor	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Although social evolutionary theory has mainly dealt with helping behaviors , competition for limited resources creates ecological conditions in which an actor may benefit from expressing behaviors that reduce the vital rates of neighbors .
	manualset3
214763	7	419717	7	NULL	NULL	NULL	NULL	 behaviors	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although social evolutionary theory has mainly dealt with helping behaviors , competition for limited resources creates ecological conditions in which an actor may benefit from expressing behaviors that reduce the vital rates of neighbors .
	manualset3
214764	8	419717	7	NULL	NULL	0	NULL	 vital rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although social evolutionary theory has mainly dealt with helping behaviors , competition for limited resources creates ecological conditions in which an actor may benefit from expressing behaviors that reduce the vital rates of neighbors .
	manualset3
215486	9	419717	7	NULL	NULL	0	NULL	neighbors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although social evolutionary theory has mainly dealt with helping behaviors , competition for limited resources creates ecological conditions in which an actor may benefit from expressing behaviors that reduce the vital rates of neighbors .
	manualset3
214765	1	419718	7	NULL	NULL	0	NULL	anemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We found that anemia is associated with increased long-term mortality rates in patients who have diastolic heart failure .
	manualset3
214766	2	419718	7	NULL	NULL	0	NULL	increased long-term mortality rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We found that anemia is associated with increased long-term mortality rates in patients who have diastolic heart failure .
	manualset3
214767	3	419718	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We found that anemia is associated with increased long-term mortality rates in patients who have diastolic heart failure .
	manualset3
214768	4	419718	7	NULL	NULL	0	NULL	diastolic heart failure .	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We found that anemia is associated with increased long-term mortality rates in patients who have diastolic heart failure .
	manualset3
214769	1	419719	7	NULL	NULL	0	NULL	Transcriptional activators	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcriptional activators in prokaryotes have been shown to stimulate different steps in the initiation process including the initial binding of RNA polymerase ( RNAP ) to the promoter and a postbinding step known as the isomerization step .
	manualset3
214770	2	419719	7	NULL	NULL	0	NULL	prokaryotes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcriptional activators in prokaryotes have been shown to stimulate different steps in the initiation process including the initial binding of RNA polymerase ( RNAP ) to the promoter and a postbinding step known as the isomerization step .
	manualset3
214771	3	419719	7	NULL	NULL	0	NULL	different steps	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcriptional activators in prokaryotes have been shown to stimulate different steps in the initiation process including the initial binding of RNA polymerase ( RNAP ) to the promoter and a postbinding step known as the isomerization step .
	manualset3
214772	4	419719	7	NULL	NULL	0	NULL	initiation process	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcriptional activators in prokaryotes have been shown to stimulate different steps in the initiation process including the initial binding of RNA polymerase ( RNAP ) to the promoter and a postbinding step known as the isomerization step .
	manualset3
214773	5	419719	7	NULL	NULL	0	NULL	initial binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcriptional activators in prokaryotes have been shown to stimulate different steps in the initiation process including the initial binding of RNA polymerase ( RNAP ) to the promoter and a postbinding step known as the isomerization step .
	manualset3
214774	6	419719	7	NULL	NULL	0	NULL	RNA polymerase ( RNAP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcriptional activators in prokaryotes have been shown to stimulate different steps in the initiation process including the initial binding of RNA polymerase ( RNAP ) to the promoter and a postbinding step known as the isomerization step .
	manualset3
214775	7	419719	7	NULL	NULL	0	NULL	promoter 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcriptional activators in prokaryotes have been shown to stimulate different steps in the initiation process including the initial binding of RNA polymerase ( RNAP ) to the promoter and a postbinding step known as the isomerization step .
	manualset3
214776	8	419719	7	NULL	NULL	0	NULL	postbinding step	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcriptional activators in prokaryotes have been shown to stimulate different steps in the initiation process including the initial binding of RNA polymerase ( RNAP ) to the promoter and a postbinding step known as the isomerization step .
	manualset3
214777	9	419719	7	NULL	NULL	0	NULL	isomerization step	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transcriptional activators in prokaryotes have been shown to stimulate different steps in the initiation process including the initial binding of RNA polymerase ( RNAP ) to the promoter and a postbinding step known as the isomerization step .
	manualset3
214778	1	419720	7	NULL	NULL	0	NULL	 residual deficits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We consider her residual deficits in the light of Farah 's ( 1990 ) theoretical framework ; this proposes that associative agnosia could be due to a disconnection syndrome , a loss of stored visual representations or to the loss of knowledge of how to perceive objects .
	manualset3
214779	2	419720	7	NULL	NULL	0	NULL	 light	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We consider her residual deficits in the light of Farah 's ( 1990 ) theoretical framework ; this proposes that associative agnosia could be due to a disconnection syndrome , a loss of stored visual representations or to the loss of knowledge of how to perceive objects .
	manualset3
214780	3	419720	7	NULL	NULL	0	NULL	Farah 's ( 1990 ) theoretical framework	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	We consider her residual deficits in the light of Farah 's ( 1990 ) theoretical framework ; this proposes that associative agnosia could be due to a disconnection syndrome , a loss of stored visual representations or to the loss of knowledge of how to perceive objects .
	manualset3
214781	4	419720	7	NULL	NULL	0	NULL	associative agnosia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We consider her residual deficits in the light of Farah 's ( 1990 ) theoretical framework ; this proposes that associative agnosia could be due to a disconnection syndrome , a loss of stored visual representations or to the loss of knowledge of how to perceive objects .
	manualset3
214782	5	419720	7	NULL	NULL	0	NULL	disconnection syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We consider her residual deficits in the light of Farah 's ( 1990 ) theoretical framework ; this proposes that associative agnosia could be due to a disconnection syndrome , a loss of stored visual representations or to the loss of knowledge of how to perceive objects .
	manualset3
214783	6	419720	7	NULL	NULL	NULL	NULL	 loss of stored visual representations	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We consider her residual deficits in the light of Farah 's ( 1990 ) theoretical framework ; this proposes that associative agnosia could be due to a disconnection syndrome , a loss of stored visual representations or to the loss of knowledge of how to perceive objects .
	manualset3
214784	7	419720	7	NULL	NULL	NULL	NULL	 loss of knowledge	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We consider her residual deficits in the light of Farah 's ( 1990 ) theoretical framework ; this proposes that associative agnosia could be due to a disconnection syndrome , a loss of stored visual representations or to the loss of knowledge of how to perceive objects .
	manualset3
214785	8	419720	7	NULL	NULL	0	NULL	perceive objects 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We consider her residual deficits in the light of Farah 's ( 1990 ) theoretical framework ; this proposes that associative agnosia could be due to a disconnection syndrome , a loss of stored visual representations or to the loss of knowledge of how to perceive objects .
	manualset3
214786	1	419721	7	NULL	NULL	0	NULL	Mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the cystic fibrosis transmembrane conductance regulator ( CFTR ) are responsible for cystic fibrosis .
	manualset3
214787	2	419721	7	NULL	NULL	0	NULL	cystic fibrosis transmembrane conductance regulator ( CFTR )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the cystic fibrosis transmembrane conductance regulator ( CFTR ) are responsible for cystic fibrosis .
	manualset3
214788	3	419721	7	NULL	NULL	0	NULL	cystic fibrosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the cystic fibrosis transmembrane conductance regulator ( CFTR ) are responsible for cystic fibrosis .
	manualset3
214789	1	419722	7	NULL	NULL	0	NULL	 effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the effect of D-1 and D-2 agonists and antagonists were differentiated in drug discrimination studies , using the cue induced by the D-1 agonist SK & F 38393 or by the D-2 agonist ( - ) - NPA versus saline .
	manualset3
214790	2	419722	7	NULL	NULL	NULL	NULL	D-1 agonists	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , the effect of D-1 and D-2 agonists and antagonists were differentiated in drug discrimination studies , using the cue induced by the D-1 agonist SK & F 38393 or by the D-2 agonist ( - ) - NPA versus saline .
	manualset3
214791	3	419722	7	NULL	NULL	NULL	NULL	D-2 agonists	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , the effect of D-1 and D-2 agonists and antagonists were differentiated in drug discrimination studies , using the cue induced by the D-1 agonist SK & F 38393 or by the D-2 agonist ( - ) - NPA versus saline .
	manualset3
214792	4	419722	7	NULL	NULL	NULL	NULL	D-1 antagonists	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , the effect of D-1 and D-2 agonists and antagonists were differentiated in drug discrimination studies , using the cue induced by the D-1 agonist SK & F 38393 or by the D-2 agonist ( - ) - NPA versus saline .
	manualset3
214793	5	419722	7	NULL	NULL	NULL	NULL	D-2 antagonists	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , the effect of D-1 and D-2 agonists and antagonists were differentiated in drug discrimination studies , using the cue induced by the D-1 agonist SK & F 38393 or by the D-2 agonist ( - ) - NPA versus saline .
	manualset3
214794	6	419722	7	NULL	NULL	0	NULL	drug discrimination studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the effect of D-1 and D-2 agonists and antagonists were differentiated in drug discrimination studies , using the cue induced by the D-1 agonist SK & F 38393 or by the D-2 agonist ( - ) - NPA versus saline .
	manualset3
214795	7	419722	7	NULL	NULL	0	NULL	cue	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the effect of D-1 and D-2 agonists and antagonists were differentiated in drug discrimination studies , using the cue induced by the D-1 agonist SK & F 38393 or by the D-2 agonist ( - ) - NPA versus saline .
	manualset3
214796	8	419722	7	NULL	NULL	0	NULL	D-1 agonist SK & F 38393	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the effect of D-1 and D-2 agonists and antagonists were differentiated in drug discrimination studies , using the cue induced by the D-1 agonist SK & F 38393 or by the D-2 agonist ( - ) - NPA versus saline .
	manualset3
214797	9	419722	7	NULL	NULL	0	NULL	D-2 agonist ( - ) - NPA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the effect of D-1 and D-2 agonists and antagonists were differentiated in drug discrimination studies , using the cue induced by the D-1 agonist SK & F 38393 or by the D-2 agonist ( - ) - NPA versus saline .
	manualset3
214798	10	419722	7	NULL	NULL	0	NULL	saline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the effect of D-1 and D-2 agonists and antagonists were differentiated in drug discrimination studies , using the cue induced by the D-1 agonist SK & F 38393 or by the D-2 agonist ( - ) - NPA versus saline .
	manualset3
214799	1	419723	7	NULL	NULL	NULL	NULL	otosclerotic stapes footplate	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The otosclerotic stapes footplate exhibits higher activities of cathepsin D and H and collagenase-like peptidase than those of normal cortical bone .
	manualset3
214800	2	419723	7	NULL	NULL	0	NULL	higher activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The otosclerotic stapes footplate exhibits higher activities of cathepsin D and H and collagenase-like peptidase than those of normal cortical bone .
	manualset3
214801	3	419723	7	NULL	NULL	0	NULL	cathepsin D	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The otosclerotic stapes footplate exhibits higher activities of cathepsin D and H and collagenase-like peptidase than those of normal cortical bone .
	manualset3
214802	4	419723	7	NULL	NULL	0	NULL	cathepsin H	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The otosclerotic stapes footplate exhibits higher activities of cathepsin D and H and collagenase-like peptidase than those of normal cortical bone .
	manualset3
214803	5	419723	7	NULL	NULL	0	NULL	collagenase-like peptidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The otosclerotic stapes footplate exhibits higher activities of cathepsin D and H and collagenase-like peptidase than those of normal cortical bone .
	manualset3
214804	6	419723	7	NULL	NULL	0	NULL	normal cortical bone	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The otosclerotic stapes footplate exhibits higher activities of cathepsin D and H and collagenase-like peptidase than those of normal cortical bone .
	manualset3
214805	1	419724	7	NULL	NULL	0	NULL	Donor heart preservation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Donor heart preservation with the potassium channel opener pinacidil : comparison with University of Wisconsin and St. Thomas ' solution .
	manualset3
214806	2	419724	7	NULL	NULL	0	NULL	potassium channel opener	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Donor heart preservation with the potassium channel opener pinacidil : comparison with University of Wisconsin and St. Thomas ' solution .
	manualset3
214807	3	419724	7	NULL	NULL	0	NULL	pinacidil	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Donor heart preservation with the potassium channel opener pinacidil : comparison with University of Wisconsin and St. Thomas ' solution .
	manualset3
214808	4	419724	7	NULL	NULL	0	NULL	comparison	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Donor heart preservation with the potassium channel opener pinacidil : comparison with University of Wisconsin and St. Thomas ' solution .
	manualset3
214809	5	419724	7	NULL	NULL	0	NULL	University of Wisconsin	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Donor heart preservation with the potassium channel opener pinacidil : comparison with University of Wisconsin and St. Thomas ' solution .
	manualset3
214810	6	419724	7	NULL	NULL	0	NULL	 St. Thomas ' solution	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Donor heart preservation with the potassium channel opener pinacidil : comparison with University of Wisconsin and St. Thomas ' solution .
	manualset3
214811	1	419725	7	NULL	NULL	0	NULL	International Union Against Tuberculosis and Lung Diseases ( IUATLD )	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some of the International Union Against Tuberculosis and Lung Diseases ( IUATLD ) criteria for discontinuation of BCG vaccination have been fulfilled , current TB epidemiological situation in S & M requires continuation of BCG vaccination at birth .
	manualset3
214812	2	419725	7	NULL	NULL	0	NULL	discontinuation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some of the International Union Against Tuberculosis and Lung Diseases ( IUATLD ) criteria for discontinuation of BCG vaccination have been fulfilled , current TB epidemiological situation in S & M requires continuation of BCG vaccination at birth .
	manualset3
214813	3	419725	7	NULL	NULL	0	NULL	BCG vaccination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some of the International Union Against Tuberculosis and Lung Diseases ( IUATLD ) criteria for discontinuation of BCG vaccination have been fulfilled , current TB epidemiological situation in S & M requires continuation of BCG vaccination at birth .
	manualset3
214814	4	419725	7	NULL	NULL	0	NULL	TB epidemiological situation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some of the International Union Against Tuberculosis and Lung Diseases ( IUATLD ) criteria for discontinuation of BCG vaccination have been fulfilled , current TB epidemiological situation in S & M requires continuation of BCG vaccination at birth .
	manualset3
214815	5	419725	7	NULL	NULL	0	NULL	 S & M	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some of the International Union Against Tuberculosis and Lung Diseases ( IUATLD ) criteria for discontinuation of BCG vaccination have been fulfilled , current TB epidemiological situation in S & M requires continuation of BCG vaccination at birth .
	manualset3
214816	6	419725	7	NULL	NULL	0	NULL	continuation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some of the International Union Against Tuberculosis and Lung Diseases ( IUATLD ) criteria for discontinuation of BCG vaccination have been fulfilled , current TB epidemiological situation in S & M requires continuation of BCG vaccination at birth .
	manualset3
214817	7	419725	7	NULL	NULL	0	NULL	BCG vaccination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some of the International Union Against Tuberculosis and Lung Diseases ( IUATLD ) criteria for discontinuation of BCG vaccination have been fulfilled , current TB epidemiological situation in S & M requires continuation of BCG vaccination at birth .
	manualset3
214818	8	419725	7	NULL	NULL	0	NULL	 birth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some of the International Union Against Tuberculosis and Lung Diseases ( IUATLD ) criteria for discontinuation of BCG vaccination have been fulfilled , current TB epidemiological situation in S & M requires continuation of BCG vaccination at birth .
	manualset3
214819	1	419726	7	NULL	NULL	0	NULL	single dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A single dose of AF-16 maintained the raised ICP after a TBI lowered during 3-9 h. The AF protein , enriched in egg yolk , similarly lowered the post-traumatically raised ICP in rats .
	manualset3
214820	2	419726	7	NULL	NULL	0	NULL	AF-16	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	A single dose of AF-16 maintained the raised ICP after a TBI lowered during 3-9 h. The AF protein , enriched in egg yolk , similarly lowered the post-traumatically raised ICP in rats .
	manualset3
214821	3	419726	7	NULL	NULL	0	NULL	ICP	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A single dose of AF-16 maintained the raised ICP after a TBI lowered during 3-9 h. The AF protein , enriched in egg yolk , similarly lowered the post-traumatically raised ICP in rats .
	manualset3
214822	4	419726	7	NULL	NULL	0	NULL	TBI 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A single dose of AF-16 maintained the raised ICP after a TBI lowered during 3-9 h. The AF protein , enriched in egg yolk , similarly lowered the post-traumatically raised ICP in rats .
	manualset3
214823	5	419726	7	NULL	NULL	0	NULL	3-9 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A single dose of AF-16 maintained the raised ICP after a TBI lowered during 3-9 h. The AF protein , enriched in egg yolk , similarly lowered the post-traumatically raised ICP in rats .
	manualset3
214824	6	419726	7	NULL	NULL	0	NULL	AF protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A single dose of AF-16 maintained the raised ICP after a TBI lowered during 3-9 h. The AF protein , enriched in egg yolk , similarly lowered the post-traumatically raised ICP in rats .
	manualset3
214825	7	419726	7	NULL	NULL	0	NULL	egg yolk	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A single dose of AF-16 maintained the raised ICP after a TBI lowered during 3-9 h. The AF protein , enriched in egg yolk , similarly lowered the post-traumatically raised ICP in rats .
	manualset3
214826	8	419726	7	NULL	NULL	0	NULL	post-traumatically raised ICP	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A single dose of AF-16 maintained the raised ICP after a TBI lowered during 3-9 h. The AF protein , enriched in egg yolk , similarly lowered the post-traumatically raised ICP in rats .
	manualset3
214827	9	419726	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A single dose of AF-16 maintained the raised ICP after a TBI lowered during 3-9 h. The AF protein , enriched in egg yolk , similarly lowered the post-traumatically raised ICP in rats .
	manualset3
214828	1	419727	7	NULL	NULL	0	NULL	activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity was reduced by pretreatment of lymph donors with indomethacin or soybean trypsin inhibitor .
	manualset3
214829	2	419727	7	NULL	NULL	0	NULL	pretreatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity was reduced by pretreatment of lymph donors with indomethacin or soybean trypsin inhibitor .
	manualset3
214830	3	419727	7	NULL	NULL	0	NULL	lymph donors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity was reduced by pretreatment of lymph donors with indomethacin or soybean trypsin inhibitor .
	manualset3
214831	4	419727	7	NULL	NULL	0	NULL	indomethacin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity was reduced by pretreatment of lymph donors with indomethacin or soybean trypsin inhibitor .
	manualset3
214832	5	419727	7	NULL	NULL	0	NULL	soybean trypsin inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity was reduced by pretreatment of lymph donors with indomethacin or soybean trypsin inhibitor .
	manualset3
214833	1	419728	7	NULL	NULL	0	NULL	ERKs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , ERKs activated by heterotrimeric G protein-independent mechanisms fail to phosphorylate nuclear targets due to lack of inhibition of Crm-1-induced nuclear export of ERKs .
	manualset3
214834	2	419728	7	NULL	NULL	0	NULL	heterotrimeric G protein-independent mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , ERKs activated by heterotrimeric G protein-independent mechanisms fail to phosphorylate nuclear targets due to lack of inhibition of Crm-1-induced nuclear export of ERKs .
	manualset3
214835	3	419728	7	NULL	NULL	0	NULL	nuclear targets	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , ERKs activated by heterotrimeric G protein-independent mechanisms fail to phosphorylate nuclear targets due to lack of inhibition of Crm-1-induced nuclear export of ERKs .
	manualset3
214836	4	419728	7	NULL	NULL	0	NULL	inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , ERKs activated by heterotrimeric G protein-independent mechanisms fail to phosphorylate nuclear targets due to lack of inhibition of Crm-1-induced nuclear export of ERKs .
	manualset3
214837	5	419728	7	NULL	NULL	0	NULL	Crm-1-induced nuclear export	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , ERKs activated by heterotrimeric G protein-independent mechanisms fail to phosphorylate nuclear targets due to lack of inhibition of Crm-1-induced nuclear export of ERKs .
	manualset3
214838	6	419728	7	NULL	NULL	0	NULL	ERKs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Interestingly , ERKs activated by heterotrimeric G protein-independent mechanisms fail to phosphorylate nuclear targets due to lack of inhibition of Crm-1-induced nuclear export of ERKs .
	manualset3
214839	1	419729	7	NULL	NULL	0	NULL	apoptosis genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , apoptosis genes are differentially co-expressed between humans and chimpanzees .
	manualset3
214840	2	419729	7	NULL	NULL	0	NULL	 humans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , apoptosis genes are differentially co-expressed between humans and chimpanzees .
	manualset3
214841	3	419729	7	NULL	NULL	0	NULL	chimpanzees	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , apoptosis genes are differentially co-expressed between humans and chimpanzees .
	manualset3
214842	1	419730	7	NULL	NULL	0	NULL	 lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This lesion could not be reproduced if the EAE cells were replaced by EAE serum or by irrelevantly immunized cells , or if their activity was foiled by specific `` desensitization '' or by use of histoincompatible recipients .
	manualset3
214843	2	419730	7	NULL	NULL	0	NULL	EAE cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	This lesion could not be reproduced if the EAE cells were replaced by EAE serum or by irrelevantly immunized cells , or if their activity was foiled by specific `` desensitization '' or by use of histoincompatible recipients .
	manualset3
214844	3	419730	7	NULL	NULL	0	NULL	EAE serum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This lesion could not be reproduced if the EAE cells were replaced by EAE serum or by irrelevantly immunized cells , or if their activity was foiled by specific `` desensitization '' or by use of histoincompatible recipients .
	manualset3
214845	4	419730	7	NULL	NULL	0	NULL	irrelevantly immunized cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	This lesion could not be reproduced if the EAE cells were replaced by EAE serum or by irrelevantly immunized cells , or if their activity was foiled by specific `` desensitization '' or by use of histoincompatible recipients .
	manualset3
214846	5	419730	7	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This lesion could not be reproduced if the EAE cells were replaced by EAE serum or by irrelevantly immunized cells , or if their activity was foiled by specific `` desensitization '' or by use of histoincompatible recipients .
	manualset3
214847	6	419730	7	NULL	NULL	0	NULL	`` desensitization '' 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This lesion could not be reproduced if the EAE cells were replaced by EAE serum or by irrelevantly immunized cells , or if their activity was foiled by specific `` desensitization '' or by use of histoincompatible recipients .
	manualset3
214848	7	419730	7	NULL	NULL	0	NULL	histoincompatible recipients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This lesion could not be reproduced if the EAE cells were replaced by EAE serum or by irrelevantly immunized cells , or if their activity was foiled by specific `` desensitization '' or by use of histoincompatible recipients .
	manualset3
214852	1	419731	7	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some research has been conducted to document the effect of these programs on such variables as absenteeism and disciplinary action , little information is available regarding compliance with clinical recommendations , ie , initiating and remaining in prescribed treatment .
	manualset3
214853	2	419731	7	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some research has been conducted to document the effect of these programs on such variables as absenteeism and disciplinary action , little information is available regarding compliance with clinical recommendations , ie , initiating and remaining in prescribed treatment .
	manualset3
214854	3	419731	7	NULL	NULL	0	NULL	programs	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some research has been conducted to document the effect of these programs on such variables as absenteeism and disciplinary action , little information is available regarding compliance with clinical recommendations , ie , initiating and remaining in prescribed treatment .
	manualset3
214855	4	419731	7	NULL	NULL	0	NULL	variables	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some research has been conducted to document the effect of these programs on such variables as absenteeism and disciplinary action , little information is available regarding compliance with clinical recommendations , ie , initiating and remaining in prescribed treatment .
	manualset3
214856	5	419731	7	NULL	NULL	0	NULL	absenteeism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some research has been conducted to document the effect of these programs on such variables as absenteeism and disciplinary action , little information is available regarding compliance with clinical recommendations , ie , initiating and remaining in prescribed treatment .
	manualset3
214857	6	419731	7	NULL	NULL	0	NULL	disciplinary action	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some research has been conducted to document the effect of these programs on such variables as absenteeism and disciplinary action , little information is available regarding compliance with clinical recommendations , ie , initiating and remaining in prescribed treatment .
	manualset3
214858	7	419731	7	NULL	NULL	0	NULL	little information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some research has been conducted to document the effect of these programs on such variables as absenteeism and disciplinary action , little information is available regarding compliance with clinical recommendations , ie , initiating and remaining in prescribed treatment .
	manualset3
214859	8	419731	7	NULL	NULL	0	NULL	compliance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some research has been conducted to document the effect of these programs on such variables as absenteeism and disciplinary action , little information is available regarding compliance with clinical recommendations , ie , initiating and remaining in prescribed treatment .
	manualset3
214860	9	419731	7	NULL	NULL	0	NULL	clinical recommendations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some research has been conducted to document the effect of these programs on such variables as absenteeism and disciplinary action , little information is available regarding compliance with clinical recommendations , ie , initiating and remaining in prescribed treatment .
	manualset3
214861	10	419731	7	NULL	NULL	0	NULL	 initiating	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some research has been conducted to document the effect of these programs on such variables as absenteeism and disciplinary action , little information is available regarding compliance with clinical recommendations , ie , initiating and remaining in prescribed treatment .
	manualset3
214862	11	419731	7	NULL	NULL	0	NULL	 remaining 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some research has been conducted to document the effect of these programs on such variables as absenteeism and disciplinary action , little information is available regarding compliance with clinical recommendations , ie , initiating and remaining in prescribed treatment .
	manualset3
214863	12	419731	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some research has been conducted to document the effect of these programs on such variables as absenteeism and disciplinary action , little information is available regarding compliance with clinical recommendations , ie , initiating and remaining in prescribed treatment .
	manualset3
214864	1	419732	7	NULL	NULL	0	NULL	 suppression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since suppression of arrhythmia has not yet been proven to reduce mortality , care must be taken in evaluating the risk-benefit ratio when prescribing therapy , particularly for patients with less malignant arrhythmias .
	manualset3
214865	2	419732	7	NULL	NULL	0	NULL	arrhythmia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Since suppression of arrhythmia has not yet been proven to reduce mortality , care must be taken in evaluating the risk-benefit ratio when prescribing therapy , particularly for patients with less malignant arrhythmias .
	manualset3
214866	3	419732	7	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since suppression of arrhythmia has not yet been proven to reduce mortality , care must be taken in evaluating the risk-benefit ratio when prescribing therapy , particularly for patients with less malignant arrhythmias .
	manualset3
214867	4	419732	7	NULL	NULL	0	NULL	care	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since suppression of arrhythmia has not yet been proven to reduce mortality , care must be taken in evaluating the risk-benefit ratio when prescribing therapy , particularly for patients with less malignant arrhythmias .
	manualset3
214868	5	419732	7	NULL	NULL	0	NULL	risk-benefit ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since suppression of arrhythmia has not yet been proven to reduce mortality , care must be taken in evaluating the risk-benefit ratio when prescribing therapy , particularly for patients with less malignant arrhythmias .
	manualset3
214869	6	419732	7	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Since suppression of arrhythmia has not yet been proven to reduce mortality , care must be taken in evaluating the risk-benefit ratio when prescribing therapy , particularly for patients with less malignant arrhythmias .
	manualset3
214870	7	419732	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since suppression of arrhythmia has not yet been proven to reduce mortality , care must be taken in evaluating the risk-benefit ratio when prescribing therapy , particularly for patients with less malignant arrhythmias .
	manualset3
214871	8	419732	7	NULL	NULL	0	NULL	less malignant arrhythmias	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Since suppression of arrhythmia has not yet been proven to reduce mortality , care must be taken in evaluating the risk-benefit ratio when prescribing therapy , particularly for patients with less malignant arrhythmias .
	manualset3
214872	1	419733	7	NULL	NULL	0	NULL	different modes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the different modes of LH-RH administration which all caused 3-4 fold elevations of the mean endogenous luteinizing hormone ( LH ) concentrations and 1.7-2 fold elevations of the mean follicle-stimulating hormone ( FSH ) serum levels , an overt increase of the mean testosterone ( T ) levels was noticed up to 1.5 X the baseline value .
	manualset3
214873	2	419733	7	NULL	NULL	0	NULL	LH-RH administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the different modes of LH-RH administration which all caused 3-4 fold elevations of the mean endogenous luteinizing hormone ( LH ) concentrations and 1.7-2 fold elevations of the mean follicle-stimulating hormone ( FSH ) serum levels , an overt increase of the mean testosterone ( T ) levels was noticed up to 1.5 X the baseline value .
	manualset3
214874	3	419733	7	NULL	NULL	NULL	NULL	3-4 fold elevations	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following the different modes of LH-RH administration which all caused 3-4 fold elevations of the mean endogenous luteinizing hormone ( LH ) concentrations and 1.7-2 fold elevations of the mean follicle-stimulating hormone ( FSH ) serum levels , an overt increase of the mean testosterone ( T ) levels was noticed up to 1.5 X the baseline value .
	manualset3
214875	4	419733	7	NULL	NULL	0	NULL	mean endogenous luteinizing hormone ( LH ) concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the different modes of LH-RH administration which all caused 3-4 fold elevations of the mean endogenous luteinizing hormone ( LH ) concentrations and 1.7-2 fold elevations of the mean follicle-stimulating hormone ( FSH ) serum levels , an overt increase of the mean testosterone ( T ) levels was noticed up to 1.5 X the baseline value .
	manualset3
214876	5	419733	7	NULL	NULL	NULL	NULL	1.7-2 fold elevations	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following the different modes of LH-RH administration which all caused 3-4 fold elevations of the mean endogenous luteinizing hormone ( LH ) concentrations and 1.7-2 fold elevations of the mean follicle-stimulating hormone ( FSH ) serum levels , an overt increase of the mean testosterone ( T ) levels was noticed up to 1.5 X the baseline value .
	manualset3
214877	6	419733	7	NULL	NULL	0	NULL	mean follicle-stimulating hormone ( FSH ) serum levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the different modes of LH-RH administration which all caused 3-4 fold elevations of the mean endogenous luteinizing hormone ( LH ) concentrations and 1.7-2 fold elevations of the mean follicle-stimulating hormone ( FSH ) serum levels , an overt increase of the mean testosterone ( T ) levels was noticed up to 1.5 X the baseline value .
	manualset3
214878	7	419733	7	NULL	NULL	NULL	NULL	overt increase	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following the different modes of LH-RH administration which all caused 3-4 fold elevations of the mean endogenous luteinizing hormone ( LH ) concentrations and 1.7-2 fold elevations of the mean follicle-stimulating hormone ( FSH ) serum levels , an overt increase of the mean testosterone ( T ) levels was noticed up to 1.5 X the baseline value .
	manualset3
214879	8	419733	7	NULL	NULL	0	NULL	mean testosterone ( T ) levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the different modes of LH-RH administration which all caused 3-4 fold elevations of the mean endogenous luteinizing hormone ( LH ) concentrations and 1.7-2 fold elevations of the mean follicle-stimulating hormone ( FSH ) serum levels , an overt increase of the mean testosterone ( T ) levels was noticed up to 1.5 X the baseline value .
	manualset3
214880	9	419733	7	NULL	NULL	0	NULL	1.5 X the baseline value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the different modes of LH-RH administration which all caused 3-4 fold elevations of the mean endogenous luteinizing hormone ( LH ) concentrations and 1.7-2 fold elevations of the mean follicle-stimulating hormone ( FSH ) serum levels , an overt increase of the mean testosterone ( T ) levels was noticed up to 1.5 X the baseline value .
	manualset3
214881	1	419734	7	NULL	NULL	0	NULL	order of magnitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This is an order of magnitude higher than has been reported elsewhere for soybean .
	manualset3
214882	2	419734	7	NULL	NULL	0	NULL	soybean	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	This is an order of magnitude higher than has been reported elsewhere for soybean .
	manualset3
214883	1	419735	7	NULL	NULL	0	NULL	Practical blood volume measurements	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Practical blood volume measurements with radioactive chromic chloride and iodinated human serum albumin .
	manualset3
214884	2	419735	7	NULL	NULL	0	NULL	radioactive chromic chloride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Practical blood volume measurements with radioactive chromic chloride and iodinated human serum albumin .
	manualset3
214885	3	419735	7	NULL	NULL	0	NULL	iodinated human serum albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Practical blood volume measurements with radioactive chromic chloride and iodinated human serum albumin .
	manualset3
214886	1	419736	7	NULL	NULL	0	NULL	Inspection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inspection of the conditions of work at aircraft repair plants showed that employees are impacted by a number of harmful in-plant factors including noise , infrasound , kerosene , microclimate and others .
	manualset3
214887	2	419736	7	NULL	NULL	0	NULL	conditions of work	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inspection of the conditions of work at aircraft repair plants showed that employees are impacted by a number of harmful in-plant factors including noise , infrasound , kerosene , microclimate and others .
	manualset3
214888	3	419736	7	NULL	NULL	0	NULL	aircraft repair plants	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Inspection of the conditions of work at aircraft repair plants showed that employees are impacted by a number of harmful in-plant factors including noise , infrasound , kerosene , microclimate and others .
	manualset3
214889	4	419736	7	NULL	NULL	0	NULL	employees	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Inspection of the conditions of work at aircraft repair plants showed that employees are impacted by a number of harmful in-plant factors including noise , infrasound , kerosene , microclimate and others .
	manualset3
214890	5	419736	7	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Inspection of the conditions of work at aircraft repair plants showed that employees are impacted by a number of harmful in-plant factors including noise , infrasound , kerosene , microclimate and others .
	manualset3
214891	6	419736	7	NULL	NULL	0	NULL	harmful in-plant factors	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Inspection of the conditions of work at aircraft repair plants showed that employees are impacted by a number of harmful in-plant factors including noise , infrasound , kerosene , microclimate and others .
	manualset3
214892	7	419736	7	NULL	NULL	0	NULL	noise	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Inspection of the conditions of work at aircraft repair plants showed that employees are impacted by a number of harmful in-plant factors including noise , infrasound , kerosene , microclimate and others .
	manualset3
214893	8	419736	7	NULL	NULL	0	NULL	infrasound 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Inspection of the conditions of work at aircraft repair plants showed that employees are impacted by a number of harmful in-plant factors including noise , infrasound , kerosene , microclimate and others .
	manualset3
214894	9	419736	7	NULL	NULL	0	NULL	kerosene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Inspection of the conditions of work at aircraft repair plants showed that employees are impacted by a number of harmful in-plant factors including noise , infrasound , kerosene , microclimate and others .
	manualset3
214895	10	419736	7	NULL	NULL	0	NULL	microclimate 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Inspection of the conditions of work at aircraft repair plants showed that employees are impacted by a number of harmful in-plant factors including noise , infrasound , kerosene , microclimate and others .
	manualset3
214896	1	419737	7	NULL	NULL	0	NULL	some studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some studies have supported monophyly of the subfamily , molecular analyses have produced contradictory results and there has been little agreement on relationships of cynopterines to other megabat groups .
	manualset3
214897	2	419737	7	NULL	NULL	0	NULL	monophyly 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some studies have supported monophyly of the subfamily , molecular analyses have produced contradictory results and there has been little agreement on relationships of cynopterines to other megabat groups .
	manualset3
214898	3	419737	7	NULL	NULL	0	NULL	subfamily	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some studies have supported monophyly of the subfamily , molecular analyses have produced contradictory results and there has been little agreement on relationships of cynopterines to other megabat groups .
	manualset3
214899	4	419737	7	NULL	NULL	0	NULL	molecular analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some studies have supported monophyly of the subfamily , molecular analyses have produced contradictory results and there has been little agreement on relationships of cynopterines to other megabat groups .
	manualset3
214900	5	419737	7	NULL	NULL	0	NULL	contradictory results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some studies have supported monophyly of the subfamily , molecular analyses have produced contradictory results and there has been little agreement on relationships of cynopterines to other megabat groups .
	manualset3
214901	6	419737	7	NULL	NULL	0	NULL	 agreement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some studies have supported monophyly of the subfamily , molecular analyses have produced contradictory results and there has been little agreement on relationships of cynopterines to other megabat groups .
	manualset3
214902	7	419737	7	NULL	NULL	0	NULL	 relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some studies have supported monophyly of the subfamily , molecular analyses have produced contradictory results and there has been little agreement on relationships of cynopterines to other megabat groups .
	manualset3
214903	8	419737	7	NULL	NULL	0	NULL	cynopterines	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some studies have supported monophyly of the subfamily , molecular analyses have produced contradictory results and there has been little agreement on relationships of cynopterines to other megabat groups .
	manualset3
214904	9	419737	7	NULL	NULL	0	NULL	megabat groups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some studies have supported monophyly of the subfamily , molecular analyses have produced contradictory results and there has been little agreement on relationships of cynopterines to other megabat groups .
	manualset3
214905	1	419738	7	NULL	NULL	0	NULL	Histology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Histology , ultrastructure , and chemical concentration .
	manualset3
214906	2	419738	7	NULL	NULL	0	NULL	 ultrastructure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Histology , ultrastructure , and chemical concentration .
	manualset3
214907	3	419738	7	NULL	NULL	0	NULL	chemical concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Histology , ultrastructure , and chemical concentration .
	manualset3
214908	1	419739	7	NULL	NULL	0	NULL	Exercise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Exercise significantly increased heart rate , left ventricular systolic pressure , dP/dt , segment shortening and rate of shortening , and coronary blood flow .
	manualset3
214909	2	419739	7	NULL	NULL	0	NULL	heart rate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Exercise significantly increased heart rate , left ventricular systolic pressure , dP/dt , segment shortening and rate of shortening , and coronary blood flow .
	manualset3
214910	3	419739	7	NULL	NULL	0	NULL	left ventricular systolic pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Exercise significantly increased heart rate , left ventricular systolic pressure , dP/dt , segment shortening and rate of shortening , and coronary blood flow .
	manualset3
214911	4	419739	7	NULL	NULL	0	NULL	dP/dt	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Exercise significantly increased heart rate , left ventricular systolic pressure , dP/dt , segment shortening and rate of shortening , and coronary blood flow .
	manualset3
214912	5	419739	7	NULL	NULL	0	NULL	segment shortening 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Exercise significantly increased heart rate , left ventricular systolic pressure , dP/dt , segment shortening and rate of shortening , and coronary blood flow .
	manualset3
214913	6	419739	7	NULL	NULL	0	NULL	rate of shortening	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Exercise significantly increased heart rate , left ventricular systolic pressure , dP/dt , segment shortening and rate of shortening , and coronary blood flow .
	manualset3
214914	7	419739	7	NULL	NULL	0	NULL	coronary blood flow	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Exercise significantly increased heart rate , left ventricular systolic pressure , dP/dt , segment shortening and rate of shortening , and coronary blood flow .
	manualset3
214915	1	419740	7	NULL	NULL	0	NULL	Images	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Images of a human iris contain rich texture information useful for identity authentication .
	manualset3
214916	2	419740	7	NULL	NULL	0	NULL	human iris	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Images of a human iris contain rich texture information useful for identity authentication .
	manualset3
214917	3	419740	7	NULL	NULL	0	NULL	rich texture information	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Images of a human iris contain rich texture information useful for identity authentication .
	manualset3
214918	4	419740	7	NULL	NULL	0	NULL	identity authentication	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Images of a human iris contain rich texture information useful for identity authentication .
	manualset3
214919	1	419741	7	NULL	NULL	0	NULL	isotherm	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The isotherm was able to predict BSA gradient elution from batch equilibrium data .
	manualset3
214920	2	419741	7	NULL	NULL	0	NULL	BSA gradient elution	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The isotherm was able to predict BSA gradient elution from batch equilibrium data .
	manualset3
214921	3	419741	7	NULL	NULL	0	NULL	batch equilibrium data	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The isotherm was able to predict BSA gradient elution from batch equilibrium data .
	manualset3
214922	1	419742	7	NULL	NULL	0	NULL	action 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine the action of physiological hyperinsulinemia on protein synthesis using a tracer-independent method in vivo and identify possible explanations for this discrepancy , we measured the phosphorylation of ribosomal protein S6 kinase ( P70 ( S6k ) ) and eIF4E-binding protein ( eIF4E-BP1 ) , two key proteins that regulate messenger ribonucleic acid translation and protein synthesis .
	manualset3
214923	2	419742	7	NULL	NULL	0	NULL	physiological hyperinsulinemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine the action of physiological hyperinsulinemia on protein synthesis using a tracer-independent method in vivo and identify possible explanations for this discrepancy , we measured the phosphorylation of ribosomal protein S6 kinase ( P70 ( S6k ) ) and eIF4E-binding protein ( eIF4E-BP1 ) , two key proteins that regulate messenger ribonucleic acid translation and protein synthesis .
	manualset3
214924	3	419742	7	NULL	NULL	0	NULL	protein synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine the action of physiological hyperinsulinemia on protein synthesis using a tracer-independent method in vivo and identify possible explanations for this discrepancy , we measured the phosphorylation of ribosomal protein S6 kinase ( P70 ( S6k ) ) and eIF4E-binding protein ( eIF4E-BP1 ) , two key proteins that regulate messenger ribonucleic acid translation and protein synthesis .
	manualset3
214925	4	419742	7	NULL	NULL	0	NULL	tracer-independent method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine the action of physiological hyperinsulinemia on protein synthesis using a tracer-independent method in vivo and identify possible explanations for this discrepancy , we measured the phosphorylation of ribosomal protein S6 kinase ( P70 ( S6k ) ) and eIF4E-binding protein ( eIF4E-BP1 ) , two key proteins that regulate messenger ribonucleic acid translation and protein synthesis .
	manualset3
214926	5	419742	7	NULL	NULL	0	NULL	explanations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine the action of physiological hyperinsulinemia on protein synthesis using a tracer-independent method in vivo and identify possible explanations for this discrepancy , we measured the phosphorylation of ribosomal protein S6 kinase ( P70 ( S6k ) ) and eIF4E-binding protein ( eIF4E-BP1 ) , two key proteins that regulate messenger ribonucleic acid translation and protein synthesis .
	manualset3
214927	6	419742	7	NULL	NULL	0	NULL	discrepancy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine the action of physiological hyperinsulinemia on protein synthesis using a tracer-independent method in vivo and identify possible explanations for this discrepancy , we measured the phosphorylation of ribosomal protein S6 kinase ( P70 ( S6k ) ) and eIF4E-binding protein ( eIF4E-BP1 ) , two key proteins that regulate messenger ribonucleic acid translation and protein synthesis .
	manualset3
214928	7	419742	7	NULL	NULL	0	NULL	phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine the action of physiological hyperinsulinemia on protein synthesis using a tracer-independent method in vivo and identify possible explanations for this discrepancy , we measured the phosphorylation of ribosomal protein S6 kinase ( P70 ( S6k ) ) and eIF4E-binding protein ( eIF4E-BP1 ) , two key proteins that regulate messenger ribonucleic acid translation and protein synthesis .
	manualset3
214929	8	419742	7	NULL	NULL	0	NULL	ribosomal protein S6 kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine the action of physiological hyperinsulinemia on protein synthesis using a tracer-independent method in vivo and identify possible explanations for this discrepancy , we measured the phosphorylation of ribosomal protein S6 kinase ( P70 ( S6k ) ) and eIF4E-binding protein ( eIF4E-BP1 ) , two key proteins that regulate messenger ribonucleic acid translation and protein synthesis .
	manualset3
214930	9	419742	7	NULL	NULL	0	NULL	 ( P70 ( S6k ) )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine the action of physiological hyperinsulinemia on protein synthesis using a tracer-independent method in vivo and identify possible explanations for this discrepancy , we measured the phosphorylation of ribosomal protein S6 kinase ( P70 ( S6k ) ) and eIF4E-binding protein ( eIF4E-BP1 ) , two key proteins that regulate messenger ribonucleic acid translation and protein synthesis .
	manualset3
214931	10	419742	7	NULL	NULL	0	NULL	eIF4E-binding protein ( eIF4E-BP1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine the action of physiological hyperinsulinemia on protein synthesis using a tracer-independent method in vivo and identify possible explanations for this discrepancy , we measured the phosphorylation of ribosomal protein S6 kinase ( P70 ( S6k ) ) and eIF4E-binding protein ( eIF4E-BP1 ) , two key proteins that regulate messenger ribonucleic acid translation and protein synthesis .
	manualset3
214932	11	419742	7	NULL	NULL	0	NULL	two key proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine the action of physiological hyperinsulinemia on protein synthesis using a tracer-independent method in vivo and identify possible explanations for this discrepancy , we measured the phosphorylation of ribosomal protein S6 kinase ( P70 ( S6k ) ) and eIF4E-binding protein ( eIF4E-BP1 ) , two key proteins that regulate messenger ribonucleic acid translation and protein synthesis .
	manualset3
214933	12	419742	7	NULL	NULL	0	NULL	messenger ribonucleic acid translation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine the action of physiological hyperinsulinemia on protein synthesis using a tracer-independent method in vivo and identify possible explanations for this discrepancy , we measured the phosphorylation of ribosomal protein S6 kinase ( P70 ( S6k ) ) and eIF4E-binding protein ( eIF4E-BP1 ) , two key proteins that regulate messenger ribonucleic acid translation and protein synthesis .
	manualset3
214934	13	419742	7	NULL	NULL	0	NULL	 protein synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To examine the action of physiological hyperinsulinemia on protein synthesis using a tracer-independent method in vivo and identify possible explanations for this discrepancy , we measured the phosphorylation of ribosomal protein S6 kinase ( P70 ( S6k ) ) and eIF4E-binding protein ( eIF4E-BP1 ) , two key proteins that regulate messenger ribonucleic acid translation and protein synthesis .
	manualset3
214935	1	419743	7	NULL	NULL	0	NULL	Alteration	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Alteration in DNA stability in alkaline sucrose gradients was detected by 19 hr .
	manualset3
214936	2	419743	7	NULL	NULL	0	NULL	DNA stability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Alteration in DNA stability in alkaline sucrose gradients was detected by 19 hr .
	manualset3
214937	3	419743	7	NULL	NULL	0	NULL	alkaline sucrose gradients 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Alteration in DNA stability in alkaline sucrose gradients was detected by 19 hr .
	manualset3
214938	4	419743	7	NULL	NULL	0	NULL	19 hr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Alteration in DNA stability in alkaline sucrose gradients was detected by 19 hr .
	manualset3
214939	1	419744	7	NULL	NULL	0	NULL	Spondylocarpotarsal synostosis syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Spondylocarpotarsal synostosis syndrome is a rare autosomal recessive disorder characterised by vertebral fusions , frequently manifesting as an unsegmented vertebral bar , as well as fusions of the carpal and tarsal bones .
	manualset3
214940	2	419744	7	NULL	NULL	0	NULL	rare autosomal recessive disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Spondylocarpotarsal synostosis syndrome is a rare autosomal recessive disorder characterised by vertebral fusions , frequently manifesting as an unsegmented vertebral bar , as well as fusions of the carpal and tarsal bones .
	manualset3
214941	3	419744	7	NULL	NULL	0	NULL	 vertebral fusions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Spondylocarpotarsal synostosis syndrome is a rare autosomal recessive disorder characterised by vertebral fusions , frequently manifesting as an unsegmented vertebral bar , as well as fusions of the carpal and tarsal bones .
	manualset3
214942	4	419744	7	NULL	NULL	0	NULL	unsegmented vertebral bar	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Spondylocarpotarsal synostosis syndrome is a rare autosomal recessive disorder characterised by vertebral fusions , frequently manifesting as an unsegmented vertebral bar , as well as fusions of the carpal and tarsal bones .
	manualset3
214943	5	419744	7	NULL	NULL	0	NULL	fusions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Spondylocarpotarsal synostosis syndrome is a rare autosomal recessive disorder characterised by vertebral fusions , frequently manifesting as an unsegmented vertebral bar , as well as fusions of the carpal and tarsal bones .
	manualset3
214944	6	419744	7	NULL	NULL	0	NULL	carpal bones	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Spondylocarpotarsal synostosis syndrome is a rare autosomal recessive disorder characterised by vertebral fusions , frequently manifesting as an unsegmented vertebral bar , as well as fusions of the carpal and tarsal bones .
	manualset3
214945	7	419744	7	NULL	NULL	0	NULL	 tarsal bones 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Spondylocarpotarsal synostosis syndrome is a rare autosomal recessive disorder characterised by vertebral fusions , frequently manifesting as an unsegmented vertebral bar , as well as fusions of the carpal and tarsal bones .
	manualset3
214946	1	419745	7	NULL	NULL	0	NULL	Circulating myeloid progenitor cell kinetics	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Circulating myeloid progenitor cell kinetics during hematologic recovery from chemotherapy and subsequent recombinant human granulocyte-macrophage colony-stimulating factor administration .
	manualset3
214947	2	419745	7	NULL	NULL	0	NULL	hematologic recovery	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Circulating myeloid progenitor cell kinetics during hematologic recovery from chemotherapy and subsequent recombinant human granulocyte-macrophage colony-stimulating factor administration .
	manualset3
214948	3	419745	7	NULL	NULL	0	NULL	chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Circulating myeloid progenitor cell kinetics during hematologic recovery from chemotherapy and subsequent recombinant human granulocyte-macrophage colony-stimulating factor administration .
	manualset3
214949	4	419745	7	NULL	NULL	0	NULL	recombinant human granulocyte-macrophage colony-stimulating factor administration .	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Circulating myeloid progenitor cell kinetics during hematologic recovery from chemotherapy and subsequent recombinant human granulocyte-macrophage colony-stimulating factor administration .
	manualset3
214950	1	419746	7	NULL	NULL	0	NULL	comparative resonance Raman analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative resonance Raman analysis of heme-binding PAS domains : heme iron coordination structures of the BjFixL , AxPDEA1 , EcDos , and MtDos proteins .
	manualset3
214951	2	419746	7	NULL	NULL	0	NULL	heme-binding PAS domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative resonance Raman analysis of heme-binding PAS domains : heme iron coordination structures of the BjFixL , AxPDEA1 , EcDos , and MtDos proteins .
	manualset3
214952	3	419746	7	NULL	NULL	0	NULL	heme iron coordination structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative resonance Raman analysis of heme-binding PAS domains : heme iron coordination structures of the BjFixL , AxPDEA1 , EcDos , and MtDos proteins .
	manualset3
214953	4	419746	7	NULL	NULL	0	NULL	BjFixL proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative resonance Raman analysis of heme-binding PAS domains : heme iron coordination structures of the BjFixL , AxPDEA1 , EcDos , and MtDos proteins .
	manualset3
214954	5	419746	7	NULL	NULL	0	NULL	AxPDEA1 proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative resonance Raman analysis of heme-binding PAS domains : heme iron coordination structures of the BjFixL , AxPDEA1 , EcDos , and MtDos proteins .
	manualset3
214955	6	419746	7	NULL	NULL	0	NULL	EcDos proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative resonance Raman analysis of heme-binding PAS domains : heme iron coordination structures of the BjFixL , AxPDEA1 , EcDos , and MtDos proteins .
	manualset3
214956	7	419746	7	NULL	NULL	0	NULL	MtDos proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative resonance Raman analysis of heme-binding PAS domains : heme iron coordination structures of the BjFixL , AxPDEA1 , EcDos , and MtDos proteins .
	manualset3
214957	1	419747	7	NULL	NULL	0	NULL	 understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some understanding of the mechanism by which neuronal death occurs comes from studies with scrapie-infected mice , most of the insights regarding a possible mechanism have come from cell culture models in which a synthetic peptide ( PrP106-126 ) , based on the sequence of the prion protein , has been applied to neuronal cells .
	manualset3
214958	2	419747	7	NULL	NULL	0	NULL	mechanism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some understanding of the mechanism by which neuronal death occurs comes from studies with scrapie-infected mice , most of the insights regarding a possible mechanism have come from cell culture models in which a synthetic peptide ( PrP106-126 ) , based on the sequence of the prion protein , has been applied to neuronal cells .
	manualset3
214959	3	419747	7	NULL	NULL	0	NULL	neuronal death 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some understanding of the mechanism by which neuronal death occurs comes from studies with scrapie-infected mice , most of the insights regarding a possible mechanism have come from cell culture models in which a synthetic peptide ( PrP106-126 ) , based on the sequence of the prion protein , has been applied to neuronal cells .
	manualset3
214960	4	419747	7	NULL	NULL	0	NULL	 studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some understanding of the mechanism by which neuronal death occurs comes from studies with scrapie-infected mice , most of the insights regarding a possible mechanism have come from cell culture models in which a synthetic peptide ( PrP106-126 ) , based on the sequence of the prion protein , has been applied to neuronal cells .
	manualset3
214961	5	419747	7	NULL	NULL	0	NULL	scrapie-infected mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some understanding of the mechanism by which neuronal death occurs comes from studies with scrapie-infected mice , most of the insights regarding a possible mechanism have come from cell culture models in which a synthetic peptide ( PrP106-126 ) , based on the sequence of the prion protein , has been applied to neuronal cells .
	manualset3
214962	6	419747	7	NULL	NULL	0	NULL	 insights	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some understanding of the mechanism by which neuronal death occurs comes from studies with scrapie-infected mice , most of the insights regarding a possible mechanism have come from cell culture models in which a synthetic peptide ( PrP106-126 ) , based on the sequence of the prion protein , has been applied to neuronal cells .
	manualset3
214963	7	419747	7	NULL	NULL	0	NULL	mechanism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some understanding of the mechanism by which neuronal death occurs comes from studies with scrapie-infected mice , most of the insights regarding a possible mechanism have come from cell culture models in which a synthetic peptide ( PrP106-126 ) , based on the sequence of the prion protein , has been applied to neuronal cells .
	manualset3
214964	8	419747	7	NULL	NULL	0	NULL	cell culture models	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some understanding of the mechanism by which neuronal death occurs comes from studies with scrapie-infected mice , most of the insights regarding a possible mechanism have come from cell culture models in which a synthetic peptide ( PrP106-126 ) , based on the sequence of the prion protein , has been applied to neuronal cells .
	manualset3
214965	9	419747	7	NULL	NULL	0	NULL	synthetic peptide ( PrP106-126 ) 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some understanding of the mechanism by which neuronal death occurs comes from studies with scrapie-infected mice , most of the insights regarding a possible mechanism have come from cell culture models in which a synthetic peptide ( PrP106-126 ) , based on the sequence of the prion protein , has been applied to neuronal cells .
	manualset3
214966	10	419747	7	NULL	NULL	0	NULL	 sequence 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some understanding of the mechanism by which neuronal death occurs comes from studies with scrapie-infected mice , most of the insights regarding a possible mechanism have come from cell culture models in which a synthetic peptide ( PrP106-126 ) , based on the sequence of the prion protein , has been applied to neuronal cells .
	manualset3
214967	11	419747	7	NULL	NULL	0	NULL	prion protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some understanding of the mechanism by which neuronal death occurs comes from studies with scrapie-infected mice , most of the insights regarding a possible mechanism have come from cell culture models in which a synthetic peptide ( PrP106-126 ) , based on the sequence of the prion protein , has been applied to neuronal cells .
	manualset3
214968	12	419747	7	NULL	NULL	0	NULL	neuronal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some understanding of the mechanism by which neuronal death occurs comes from studies with scrapie-infected mice , most of the insights regarding a possible mechanism have come from cell culture models in which a synthetic peptide ( PrP106-126 ) , based on the sequence of the prion protein , has been applied to neuronal cells .
	manualset3
214969	1	419748	7	NULL	NULL	0	NULL	Technetium-99m-tetrofosmin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Technetium-99m-tetrofosmin , a myocardial perfusion imaging agent was used for estimation of cardiac output by means of first-pass radionuclide angiography performed in the anterior projection .
	manualset3
214970	2	419748	7	NULL	NULL	0	NULL	myocardial perfusion imaging agent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Technetium-99m-tetrofosmin , a myocardial perfusion imaging agent was used for estimation of cardiac output by means of first-pass radionuclide angiography performed in the anterior projection .
	manualset3
214971	3	419748	7	NULL	NULL	0	NULL	estimation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Technetium-99m-tetrofosmin , a myocardial perfusion imaging agent was used for estimation of cardiac output by means of first-pass radionuclide angiography performed in the anterior projection .
	manualset3
214972	4	419748	7	NULL	NULL	0	NULL	cardiac output 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Technetium-99m-tetrofosmin , a myocardial perfusion imaging agent was used for estimation of cardiac output by means of first-pass radionuclide angiography performed in the anterior projection .
	manualset3
214973	5	419748	7	NULL	NULL	0	NULL	first-pass radionuclide angiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Technetium-99m-tetrofosmin , a myocardial perfusion imaging agent was used for estimation of cardiac output by means of first-pass radionuclide angiography performed in the anterior projection .
	manualset3
214974	6	419748	7	NULL	NULL	0	NULL	anterior projection	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Technetium-99m-tetrofosmin , a myocardial perfusion imaging agent was used for estimation of cardiac output by means of first-pass radionuclide angiography performed in the anterior projection .
	manualset3
214975	1	419749	7	NULL	NULL	0	NULL	Fourier transforms	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although Fourier transforms of such small image fields are statistically significant only at lower resolution , the data from many such image fields can be averaged at the calculated positions of high-resolution reciprocal lattice points to give accurate phases .
	manualset3
214976	2	419749	7	NULL	NULL	0	NULL	small image fields	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Although Fourier transforms of such small image fields are statistically significant only at lower resolution , the data from many such image fields can be averaged at the calculated positions of high-resolution reciprocal lattice points to give accurate phases .
	manualset3
214977	3	419749	7	NULL	NULL	0	NULL	 lower resolution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although Fourier transforms of such small image fields are statistically significant only at lower resolution , the data from many such image fields can be averaged at the calculated positions of high-resolution reciprocal lattice points to give accurate phases .
	manualset3
214978	4	419749	7	NULL	NULL	0	NULL	 data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Although Fourier transforms of such small image fields are statistically significant only at lower resolution , the data from many such image fields can be averaged at the calculated positions of high-resolution reciprocal lattice points to give accurate phases .
	manualset3
214979	5	419749	7	NULL	NULL	0	NULL	 image fields	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Although Fourier transforms of such small image fields are statistically significant only at lower resolution , the data from many such image fields can be averaged at the calculated positions of high-resolution reciprocal lattice points to give accurate phases .
	manualset3
214980	6	419749	7	NULL	NULL	0	NULL	calculated positions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although Fourier transforms of such small image fields are statistically significant only at lower resolution , the data from many such image fields can be averaged at the calculated positions of high-resolution reciprocal lattice points to give accurate phases .
	manualset3
214981	7	419749	7	NULL	NULL	0	NULL	high-resolution reciprocal lattice points	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Although Fourier transforms of such small image fields are statistically significant only at lower resolution , the data from many such image fields can be averaged at the calculated positions of high-resolution reciprocal lattice points to give accurate phases .
	manualset3
214982	8	419749	7	NULL	NULL	0	NULL	accurate phases	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although Fourier transforms of such small image fields are statistically significant only at lower resolution , the data from many such image fields can be averaged at the calculated positions of high-resolution reciprocal lattice points to give accurate phases .
	manualset3
214983	1	419750	7	NULL	NULL	0	NULL	protein stability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein stability , Ser ( 392 ) phosphorylation and Lys ( 373 ) / Lys ( 382 ) acetylation of p53 were enhanced by MG132 .
	manualset3
214984	2	419750	7	NULL	NULL	0	NULL	Ser ( 392 ) phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein stability , Ser ( 392 ) phosphorylation and Lys ( 373 ) / Lys ( 382 ) acetylation of p53 were enhanced by MG132 .
	manualset3
214985	3	419750	7	NULL	NULL	0	NULL	Lys ( 373 ) / Lys ( 382 ) acetylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein stability , Ser ( 392 ) phosphorylation and Lys ( 373 ) / Lys ( 382 ) acetylation of p53 were enhanced by MG132 .
	manualset3
214986	4	419750	7	NULL	NULL	0	NULL	p53	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein stability , Ser ( 392 ) phosphorylation and Lys ( 373 ) / Lys ( 382 ) acetylation of p53 were enhanced by MG132 .
	manualset3
214987	5	419750	7	NULL	NULL	0	NULL	MG132	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The protein stability , Ser ( 392 ) phosphorylation and Lys ( 373 ) / Lys ( 382 ) acetylation of p53 were enhanced by MG132 .
	manualset3
214988	1	419751	7	NULL	NULL	0	NULL	open reading frame 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	An open reading frame of 3498 nt cDNA was amplified from pig liver mRNA by RT-PCR .
	manualset3
214989	2	419751	7	NULL	NULL	0	NULL	 3498 nt cDNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	An open reading frame of 3498 nt cDNA was amplified from pig liver mRNA by RT-PCR .
	manualset3
214990	3	419751	7	NULL	NULL	0	NULL	pig liver mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	An open reading frame of 3498 nt cDNA was amplified from pig liver mRNA by RT-PCR .
	manualset3
214991	4	419751	7	NULL	NULL	0	NULL	RT-PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An open reading frame of 3498 nt cDNA was amplified from pig liver mRNA by RT-PCR .
	manualset3
214992	1	419752	7	NULL	NULL	0	NULL	One 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One can then attempt to improve NUE in crop plants using the knowledge gained from these studies .
	manualset3
214993	2	419752	7	NULL	NULL	0	NULL	NUE	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One can then attempt to improve NUE in crop plants using the knowledge gained from these studies .
	manualset3
214994	3	419752	7	NULL	NULL	0	NULL	crop plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	One can then attempt to improve NUE in crop plants using the knowledge gained from these studies .
	manualset3
214995	4	419752	7	NULL	NULL	0	NULL	knowledge	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One can then attempt to improve NUE in crop plants using the knowledge gained from these studies .
	manualset3
214996	5	419752	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	One can then attempt to improve NUE in crop plants using the knowledge gained from these studies .
	manualset3
214997	1	419753	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results provide evidence that MDMA and its metabolite N-Me-alpha-MeDA induce toxicity to freshly isolated rat hepatocytes .
	manualset3
214998	2	419753	7	NULL	NULL	0	NULL	 evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results provide evidence that MDMA and its metabolite N-Me-alpha-MeDA induce toxicity to freshly isolated rat hepatocytes .
	manualset3
214999	3	419753	7	NULL	NULL	0	NULL	MDMA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results provide evidence that MDMA and its metabolite N-Me-alpha-MeDA induce toxicity to freshly isolated rat hepatocytes .
	manualset3
215000	4	419753	7	NULL	NULL	0	NULL	metabolite 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results provide evidence that MDMA and its metabolite N-Me-alpha-MeDA induce toxicity to freshly isolated rat hepatocytes .
	manualset3
215001	5	419753	7	NULL	NULL	0	NULL	N-Me-alpha-MeDA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results provide evidence that MDMA and its metabolite N-Me-alpha-MeDA induce toxicity to freshly isolated rat hepatocytes .
	manualset3
215002	6	419753	7	NULL	NULL	0	NULL	toxicity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results provide evidence that MDMA and its metabolite N-Me-alpha-MeDA induce toxicity to freshly isolated rat hepatocytes .
	manualset3
215003	7	419753	7	NULL	NULL	0	NULL	freshly isolated rat hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The results provide evidence that MDMA and its metabolite N-Me-alpha-MeDA induce toxicity to freshly isolated rat hepatocytes .
	manualset3
215004	1	419754	7	NULL	NULL	0	NULL	Triple rubber band ligation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Triple rubber band ligation for hemorrhoids : prospective , randomized trial of use of local anesthetic injection .
	manualset3
215005	2	419754	7	NULL	NULL	0	NULL	hemorrhoids	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Triple rubber band ligation for hemorrhoids : prospective , randomized trial of use of local anesthetic injection .
	manualset3
215006	3	419754	7	NULL	NULL	0	NULL	randomized trial 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Triple rubber band ligation for hemorrhoids : prospective , randomized trial of use of local anesthetic injection .
	manualset3
215007	4	419754	7	NULL	NULL	0	NULL	 local anesthetic injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Triple rubber band ligation for hemorrhoids : prospective , randomized trial of use of local anesthetic injection .
	manualset3
215008	5	419754	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Triple rubber band ligation for hemorrhoids : prospective , randomized trial of use of local anesthetic injection .
	manualset3
215009	1	419755	7	NULL	NULL	0	NULL	 homology	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant homology to bacterial S7 is observed especially in the C-terminal half of the protein .
	manualset3
215010	2	419755	7	NULL	NULL	0	NULL	bacterial S7	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant homology to bacterial S7 is observed especially in the C-terminal half of the protein .
	manualset3
215011	3	419755	7	NULL	NULL	0	NULL	C-terminal half	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant homology to bacterial S7 is observed especially in the C-terminal half of the protein .
	manualset3
215012	4	419755	7	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant homology to bacterial S7 is observed especially in the C-terminal half of the protein .
	manualset3
215013	1	419756	7	NULL	NULL	0	NULL	Dolichol-P	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Dolichol-P - and dolichol-P-P-linked saccharides were isolated from several trypanosomatid flagellates incubated with ( U-14C ) glucose .
	manualset3
215014	2	419756	7	NULL	NULL	0	NULL	dolichol-P-P-linked saccharides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Dolichol-P - and dolichol-P-P-linked saccharides were isolated from several trypanosomatid flagellates incubated with ( U-14C ) glucose .
	manualset3
215015	3	419756	7	NULL	NULL	0	NULL	several trypanosomatid flagellates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Dolichol-P - and dolichol-P-P-linked saccharides were isolated from several trypanosomatid flagellates incubated with ( U-14C ) glucose .
	manualset3
215016	4	419756	7	NULL	NULL	0	NULL	 ( U-14C ) glucose 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Dolichol-P - and dolichol-P-P-linked saccharides were isolated from several trypanosomatid flagellates incubated with ( U-14C ) glucose .
	manualset3
215017	1	419757	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These patients will be followed to assess which of these three markers of proliferation is of greatest prognostic value .
	manualset3
215018	2	419757	7	NULL	NULL	0	NULL	three markers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These patients will be followed to assess which of these three markers of proliferation is of greatest prognostic value .
	manualset3
215019	3	419757	7	NULL	NULL	0	NULL	proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These patients will be followed to assess which of these three markers of proliferation is of greatest prognostic value .
	manualset3
215020	4	419757	7	NULL	NULL	0	NULL	greatest prognostic value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These patients will be followed to assess which of these three markers of proliferation is of greatest prognostic value .
	manualset3
215021	1	419758	7	NULL	NULL	0	NULL	Samples	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples were from complete hydatidiform moles , partial hydatidiform moles , ectopic pregnancies , gestational age-matched normal elective pregnancy terminations ( normal pregnancies ) and gestational trophoblastic neoplasias .
	manualset3
215022	2	419758	7	NULL	NULL	NULL	NULL	complete hydatidiform moles	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Samples were from complete hydatidiform moles , partial hydatidiform moles , ectopic pregnancies , gestational age-matched normal elective pregnancy terminations ( normal pregnancies ) and gestational trophoblastic neoplasias .
	manualset3
215023	3	419758	7	NULL	NULL	0	NULL	partial hydatidiform moles	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples were from complete hydatidiform moles , partial hydatidiform moles , ectopic pregnancies , gestational age-matched normal elective pregnancy terminations ( normal pregnancies ) and gestational trophoblastic neoplasias .
	manualset3
215024	4	419758	7	NULL	NULL	0	NULL	ectopic pregnancies	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples were from complete hydatidiform moles , partial hydatidiform moles , ectopic pregnancies , gestational age-matched normal elective pregnancy terminations ( normal pregnancies ) and gestational trophoblastic neoplasias .
	manualset3
215025	5	419758	7	NULL	NULL	0	NULL	gestational age-matched normal elective pregnancy terminations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples were from complete hydatidiform moles , partial hydatidiform moles , ectopic pregnancies , gestational age-matched normal elective pregnancy terminations ( normal pregnancies ) and gestational trophoblastic neoplasias .
	manualset3
215026	6	419758	7	NULL	NULL	0	NULL	normal pregnancies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples were from complete hydatidiform moles , partial hydatidiform moles , ectopic pregnancies , gestational age-matched normal elective pregnancy terminations ( normal pregnancies ) and gestational trophoblastic neoplasias .
	manualset3
215027	7	419758	7	NULL	NULL	0	NULL	gestational trophoblastic neoplasias	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples were from complete hydatidiform moles , partial hydatidiform moles , ectopic pregnancies , gestational age-matched normal elective pregnancy terminations ( normal pregnancies ) and gestational trophoblastic neoplasias .
	manualset3
215028	1	419759	7	NULL	NULL	0	NULL	composite phylogeny	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We construct a composite phylogeny for these species , and we codify gravitational stress according to species habitat and behavior .
	manualset3
215029	2	419759	7	NULL	NULL	0	NULL	species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We construct a composite phylogeny for these species , and we codify gravitational stress according to species habitat and behavior .
	manualset3
215030	3	419759	7	NULL	NULL	0	NULL	 gravitational stress 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We construct a composite phylogeny for these species , and we codify gravitational stress according to species habitat and behavior .
	manualset3
215031	4	419759	7	NULL	NULL	0	NULL	species habitat	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We construct a composite phylogeny for these species , and we codify gravitational stress according to species habitat and behavior .
	manualset3
215032	5	419759	7	NULL	NULL	0	NULL	 behavior	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We construct a composite phylogeny for these species , and we codify gravitational stress according to species habitat and behavior .
	manualset3
215033	1	419760	7	NULL	NULL	0	NULL	Ca channel blockers	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The Ca channel blockers diltiazem and verapamil did not affect the responses .
	manualset3
215034	2	419760	7	NULL	NULL	0	NULL	diltiazem	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The Ca channel blockers diltiazem and verapamil did not affect the responses .
	manualset3
215035	3	419760	7	NULL	NULL	0	NULL	verapamil	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The Ca channel blockers diltiazem and verapamil did not affect the responses .
	manualset3
215036	4	419760	7	NULL	NULL	0	NULL	responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Ca channel blockers diltiazem and verapamil did not affect the responses .
	manualset3
215037	1	419761	7	NULL	NULL	0	NULL	 views	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some views of face perception posit independent processing of face identity and expression , recent studies suggest interactive processing of these 2 domains .
	manualset3
215038	2	419761	7	NULL	NULL	0	NULL	face perception posit independent processing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some views of face perception posit independent processing of face identity and expression , recent studies suggest interactive processing of these 2 domains .
	manualset3
215039	3	419761	7	NULL	NULL	0	NULL	 face identity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some views of face perception posit independent processing of face identity and expression , recent studies suggest interactive processing of these 2 domains .
	manualset3
215040	4	419761	7	NULL	NULL	0	NULL	expression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some views of face perception posit independent processing of face identity and expression , recent studies suggest interactive processing of these 2 domains .
	manualset3
215041	5	419761	7	NULL	NULL	0	NULL	 recent studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some views of face perception posit independent processing of face identity and expression , recent studies suggest interactive processing of these 2 domains .
	manualset3
215042	6	419761	7	NULL	NULL	0	NULL	 interactive processing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some views of face perception posit independent processing of face identity and expression , recent studies suggest interactive processing of these 2 domains .
	manualset3
215043	7	419761	7	NULL	NULL	0	NULL	2 domains	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although some views of face perception posit independent processing of face identity and expression , recent studies suggest interactive processing of these 2 domains .
	manualset3
215044	1	419762	7	NULL	NULL	0	NULL	63 donor samples 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 63 donor samples ( 61 % ) that tested negative for CMV-IgG by FIAX , there were two false-positive results in bag segments by PLA testing , one on Day 1 and the other on Day 2 of storage .
	manualset3
215045	2	419762	7	NULL	NULL	0	NULL	61 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 63 donor samples ( 61 % ) that tested negative for CMV-IgG by FIAX , there were two false-positive results in bag segments by PLA testing , one on Day 1 and the other on Day 2 of storage .
	manualset3
215046	3	419762	7	NULL	NULL	0	NULL	CMV-IgG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 63 donor samples ( 61 % ) that tested negative for CMV-IgG by FIAX , there were two false-positive results in bag segments by PLA testing , one on Day 1 and the other on Day 2 of storage .
	manualset3
215047	4	419762	7	NULL	NULL	0	NULL	 FIAX	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 63 donor samples ( 61 % ) that tested negative for CMV-IgG by FIAX , there were two false-positive results in bag segments by PLA testing , one on Day 1 and the other on Day 2 of storage .
	manualset3
215048	5	419762	7	NULL	NULL	0	NULL	two false-positive results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 63 donor samples ( 61 % ) that tested negative for CMV-IgG by FIAX , there were two false-positive results in bag segments by PLA testing , one on Day 1 and the other on Day 2 of storage .
	manualset3
215049	6	419762	7	NULL	NULL	0	NULL	bag segments	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 63 donor samples ( 61 % ) that tested negative for CMV-IgG by FIAX , there were two false-positive results in bag segments by PLA testing , one on Day 1 and the other on Day 2 of storage .
	manualset3
215050	7	419762	7	NULL	NULL	0	NULL	PLA testing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 63 donor samples ( 61 % ) that tested negative for CMV-IgG by FIAX , there were two false-positive results in bag segments by PLA testing , one on Day 1 and the other on Day 2 of storage .
	manualset3
215051	8	419762	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 63 donor samples ( 61 % ) that tested negative for CMV-IgG by FIAX , there were two false-positive results in bag segments by PLA testing , one on Day 1 and the other on Day 2 of storage .
	manualset3
215052	9	419762	7	NULL	NULL	0	NULL	Day 1	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 63 donor samples ( 61 % ) that tested negative for CMV-IgG by FIAX , there were two false-positive results in bag segments by PLA testing , one on Day 1 and the other on Day 2 of storage .
	manualset3
215053	10	419762	7	NULL	NULL	0	NULL	Day 2 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 63 donor samples ( 61 % ) that tested negative for CMV-IgG by FIAX , there were two false-positive results in bag segments by PLA testing , one on Day 1 and the other on Day 2 of storage .
	manualset3
215054	11	419762	7	NULL	NULL	0	NULL	storage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Of 63 donor samples ( 61 % ) that tested negative for CMV-IgG by FIAX , there were two false-positive results in bag segments by PLA testing , one on Day 1 and the other on Day 2 of storage .
	manualset3
215055	1	419763	7	NULL	NULL	0	NULL	Quantitative X-ray CT	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative X-ray CT has enabled the use of a computerized stem design program , which designs an optimal-fit hip stem for individual femurs .
	manualset3
215056	2	419763	7	NULL	NULL	0	NULL	computerized stem design program	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative X-ray CT has enabled the use of a computerized stem design program , which designs an optimal-fit hip stem for individual femurs .
	manualset3
215057	3	419763	7	NULL	NULL	0	NULL	optimal-fit hip stem	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative X-ray CT has enabled the use of a computerized stem design program , which designs an optimal-fit hip stem for individual femurs .
	manualset3
215058	4	419763	7	NULL	NULL	0	NULL	individual femurs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative X-ray CT has enabled the use of a computerized stem design program , which designs an optimal-fit hip stem for individual femurs .
	manualset3
216151	5	419763	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative X-ray CT has enabled the use of a computerized stem design program , which designs an optimal-fit hip stem for individual femurs .
	manualset3
215059	1	419764	7	NULL	NULL	NULL	NULL	human urocortin 2 gene 	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The human urocortin 2 gene is regulated by hypoxia : identification of a hypoxia-responsive element in the 3 ' - flanking region .
	manualset3
215060	2	419764	7	NULL	NULL	0	NULL	hypoxia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The human urocortin 2 gene is regulated by hypoxia : identification of a hypoxia-responsive element in the 3 ' - flanking region .
	manualset3
215061	3	419764	7	NULL	NULL	0	NULL	identification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The human urocortin 2 gene is regulated by hypoxia : identification of a hypoxia-responsive element in the 3 ' - flanking region .
	manualset3
215062	4	419764	7	NULL	NULL	0	NULL	hypoxia-responsive element	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The human urocortin 2 gene is regulated by hypoxia : identification of a hypoxia-responsive element in the 3 ' - flanking region .
	manualset3
215063	5	419764	7	NULL	NULL	0	NULL	3 ' - flanking region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The human urocortin 2 gene is regulated by hypoxia : identification of a hypoxia-responsive element in the 3 ' - flanking region .
	manualset3
215064	1	419765	7	NULL	NULL	0	NULL	Alanine aminopeptidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Alanine aminopeptidase and beta 2-microglobulin excretion in patients receiving vancomycin and gentamicin .
	manualset3
215065	2	419765	7	NULL	NULL	0	NULL	beta 2-microglobulin excretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Alanine aminopeptidase and beta 2-microglobulin excretion in patients receiving vancomycin and gentamicin .
	manualset3
215066	3	419765	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Alanine aminopeptidase and beta 2-microglobulin excretion in patients receiving vancomycin and gentamicin .
	manualset3
215067	4	419765	7	NULL	NULL	0	NULL	vancomycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Alanine aminopeptidase and beta 2-microglobulin excretion in patients receiving vancomycin and gentamicin .
	manualset3
215068	5	419765	7	NULL	NULL	0	NULL	gentamicin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Alanine aminopeptidase and beta 2-microglobulin excretion in patients receiving vancomycin and gentamicin .
	manualset3
215069	1	419766	7	NULL	NULL	NULL	NULL	Imiquimod 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Imiquimod in combination with meglumine antimoniate for cutaneous leishmaniasis : a randomized assessor-blind controlled trial .
	manualset3
215070	2	419766	7	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Imiquimod in combination with meglumine antimoniate for cutaneous leishmaniasis : a randomized assessor-blind controlled trial .
	manualset3
215071	3	419766	7	NULL	NULL	0	NULL	meglumine antimoniate	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Imiquimod in combination with meglumine antimoniate for cutaneous leishmaniasis : a randomized assessor-blind controlled trial .
	manualset3
215072	4	419766	7	NULL	NULL	0	NULL	cutaneous leishmaniasis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Imiquimod in combination with meglumine antimoniate for cutaneous leishmaniasis : a randomized assessor-blind controlled trial .
	manualset3
215073	5	419766	7	NULL	NULL	0	NULL	randomized assessor-blind controlled trial	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Imiquimod in combination with meglumine antimoniate for cutaneous leishmaniasis : a randomized assessor-blind controlled trial .
	manualset3
215074	1	419767	7	NULL	NULL	0	NULL	construction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the construction of the Chaohu Dam , an increase in the utilization of fertilizer and the population growth which occurred since 1960 , stable depositional conditions and increasing nutrient input resulted in a dominantly algae-derived organic matter source and high productivity .
	manualset3
215075	2	419767	7	NULL	NULL	0	NULL	Chaohu Dam	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	With the construction of the Chaohu Dam , an increase in the utilization of fertilizer and the population growth which occurred since 1960 , stable depositional conditions and increasing nutrient input resulted in a dominantly algae-derived organic matter source and high productivity .
	manualset3
215076	3	419767	7	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the construction of the Chaohu Dam , an increase in the utilization of fertilizer and the population growth which occurred since 1960 , stable depositional conditions and increasing nutrient input resulted in a dominantly algae-derived organic matter source and high productivity .
	manualset3
215077	4	419767	7	NULL	NULL	0	NULL	 utilization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the construction of the Chaohu Dam , an increase in the utilization of fertilizer and the population growth which occurred since 1960 , stable depositional conditions and increasing nutrient input resulted in a dominantly algae-derived organic matter source and high productivity .
	manualset3
215078	5	419767	7	NULL	NULL	0	NULL	fertilizer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	With the construction of the Chaohu Dam , an increase in the utilization of fertilizer and the population growth which occurred since 1960 , stable depositional conditions and increasing nutrient input resulted in a dominantly algae-derived organic matter source and high productivity .
	manualset3
215079	6	419767	7	NULL	NULL	0	NULL	population growth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	With the construction of the Chaohu Dam , an increase in the utilization of fertilizer and the population growth which occurred since 1960 , stable depositional conditions and increasing nutrient input resulted in a dominantly algae-derived organic matter source and high productivity .
	manualset3
215080	7	419767	7	NULL	NULL	NULL	NULL	1960	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	With the construction of the Chaohu Dam , an increase in the utilization of fertilizer and the population growth which occurred since 1960 , stable depositional conditions and increasing nutrient input resulted in a dominantly algae-derived organic matter source and high productivity .
	manualset3
215081	8	419767	7	NULL	NULL	0	NULL	stable depositional conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	With the construction of the Chaohu Dam , an increase in the utilization of fertilizer and the population growth which occurred since 1960 , stable depositional conditions and increasing nutrient input resulted in a dominantly algae-derived organic matter source and high productivity .
	manualset3
215082	9	419767	7	NULL	NULL	0	NULL	nutrient input	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	With the construction of the Chaohu Dam , an increase in the utilization of fertilizer and the population growth which occurred since 1960 , stable depositional conditions and increasing nutrient input resulted in a dominantly algae-derived organic matter source and high productivity .
	manualset3
215083	10	419767	7	NULL	NULL	0	NULL	dominantly algae-derived organic matter source	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	With the construction of the Chaohu Dam , an increase in the utilization of fertilizer and the population growth which occurred since 1960 , stable depositional conditions and increasing nutrient input resulted in a dominantly algae-derived organic matter source and high productivity .
	manualset3
215084	11	419767	7	NULL	NULL	0	NULL	high productivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With the construction of the Chaohu Dam , an increase in the utilization of fertilizer and the population growth which occurred since 1960 , stable depositional conditions and increasing nutrient input resulted in a dominantly algae-derived organic matter source and high productivity .
	manualset3
215085	1	419768	7	NULL	NULL	0	NULL	Evasion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Evasion of apoptosis can be caused by epigenetic silencing of caspase-8 , a key component of the extrinsic apoptosis pathway .
	manualset3
215086	2	419768	7	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Evasion of apoptosis can be caused by epigenetic silencing of caspase-8 , a key component of the extrinsic apoptosis pathway .
	manualset3
215087	3	419768	7	NULL	NULL	0	NULL	epigenetic silencing	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Evasion of apoptosis can be caused by epigenetic silencing of caspase-8 , a key component of the extrinsic apoptosis pathway .
	manualset3
215088	4	419768	7	NULL	NULL	0	NULL	caspase-8	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Evasion of apoptosis can be caused by epigenetic silencing of caspase-8 , a key component of the extrinsic apoptosis pathway .
	manualset3
215089	5	419768	7	NULL	NULL	0	NULL	component 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Evasion of apoptosis can be caused by epigenetic silencing of caspase-8 , a key component of the extrinsic apoptosis pathway .
	manualset3
215090	6	419768	7	NULL	NULL	0	NULL	extrinsic apoptosis pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Evasion of apoptosis can be caused by epigenetic silencing of caspase-8 , a key component of the extrinsic apoptosis pathway .
	manualset3
215091	1	419769	7	NULL	NULL	NULL	NULL	soybean	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although soybean is used in quite a number of African countries as a weaning food , there are still problems such as lack of technical know-how for its processing into infant foods , cultural practices which favor the use of cereal rather than legumes for weaning infants and the long cooking time .
	manualset3
215092	2	419769	7	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although soybean is used in quite a number of African countries as a weaning food , there are still problems such as lack of technical know-how for its processing into infant foods , cultural practices which favor the use of cereal rather than legumes for weaning infants and the long cooking time .
	manualset3
215093	3	419769	7	NULL	NULL	0	NULL	African countries	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Although soybean is used in quite a number of African countries as a weaning food , there are still problems such as lack of technical know-how for its processing into infant foods , cultural practices which favor the use of cereal rather than legumes for weaning infants and the long cooking time .
	manualset3
215094	4	419769	7	NULL	NULL	0	NULL	weaning food	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Although soybean is used in quite a number of African countries as a weaning food , there are still problems such as lack of technical know-how for its processing into infant foods , cultural practices which favor the use of cereal rather than legumes for weaning infants and the long cooking time .
	manualset3
215095	5	419769	7	NULL	NULL	0	NULL	problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although soybean is used in quite a number of African countries as a weaning food , there are still problems such as lack of technical know-how for its processing into infant foods , cultural practices which favor the use of cereal rather than legumes for weaning infants and the long cooking time .
	manualset3
215096	6	419769	7	NULL	NULL	0	NULL	 processing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although soybean is used in quite a number of African countries as a weaning food , there are still problems such as lack of technical know-how for its processing into infant foods , cultural practices which favor the use of cereal rather than legumes for weaning infants and the long cooking time .
	manualset3
215097	7	419769	7	NULL	NULL	0	NULL	infant foods	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Although soybean is used in quite a number of African countries as a weaning food , there are still problems such as lack of technical know-how for its processing into infant foods , cultural practices which favor the use of cereal rather than legumes for weaning infants and the long cooking time .
	manualset3
215098	8	419769	7	NULL	NULL	0	NULL	cultural practices	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although soybean is used in quite a number of African countries as a weaning food , there are still problems such as lack of technical know-how for its processing into infant foods , cultural practices which favor the use of cereal rather than legumes for weaning infants and the long cooking time .
	manualset3
215099	9	419769	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although soybean is used in quite a number of African countries as a weaning food , there are still problems such as lack of technical know-how for its processing into infant foods , cultural practices which favor the use of cereal rather than legumes for weaning infants and the long cooking time .
	manualset3
215100	10	419769	7	NULL	NULL	0	NULL	cereal	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Although soybean is used in quite a number of African countries as a weaning food , there are still problems such as lack of technical know-how for its processing into infant foods , cultural practices which favor the use of cereal rather than legumes for weaning infants and the long cooking time .
	manualset3
215101	11	419769	7	NULL	NULL	0	NULL	legumes	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Although soybean is used in quite a number of African countries as a weaning food , there are still problems such as lack of technical know-how for its processing into infant foods , cultural practices which favor the use of cereal rather than legumes for weaning infants and the long cooking time .
	manualset3
215102	12	419769	7	NULL	NULL	0	NULL	weaning infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although soybean is used in quite a number of African countries as a weaning food , there are still problems such as lack of technical know-how for its processing into infant foods , cultural practices which favor the use of cereal rather than legumes for weaning infants and the long cooking time .
	manualset3
215103	13	419769	7	NULL	NULL	0	NULL	long cooking time	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Although soybean is used in quite a number of African countries as a weaning food , there are still problems such as lack of technical know-how for its processing into infant foods , cultural practices which favor the use of cereal rather than legumes for weaning infants and the long cooking time .
	manualset3
215104	1	419770	7	NULL	NULL	0	NULL	Data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Data concerning the fate , occurrence , properties and extraction of triazines and their degradation products using different SPE techniques are tabulated and discussed .
	manualset3
215105	2	419770	7	NULL	NULL	NULL	NULL	fate 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data concerning the fate , occurrence , properties and extraction of triazines and their degradation products using different SPE techniques are tabulated and discussed .
	manualset3
215106	3	419770	7	NULL	NULL	0	NULL	extraction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Data concerning the fate , occurrence , properties and extraction of triazines and their degradation products using different SPE techniques are tabulated and discussed .
	manualset3
215107	4	419770	7	NULL	NULL	0	NULL	 triazines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Data concerning the fate , occurrence , properties and extraction of triazines and their degradation products using different SPE techniques are tabulated and discussed .
	manualset3
215108	5	419770	7	NULL	NULL	0	NULL	 degradation products	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Data concerning the fate , occurrence , properties and extraction of triazines and their degradation products using different SPE techniques are tabulated and discussed .
	manualset3
215109	6	419770	7	NULL	NULL	0	NULL	different SPE techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Data concerning the fate , occurrence , properties and extraction of triazines and their degradation products using different SPE techniques are tabulated and discussed .
	manualset3
215110	7	419770	7	NULL	NULL	0	NULL	occurrence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Data concerning the fate , occurrence , properties and extraction of triazines and their degradation products using different SPE techniques are tabulated and discussed .
	manualset3
216152	8	419770	7	NULL	NULL	0	NULL	properties	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Data concerning the fate , occurrence , properties and extraction of triazines and their degradation products using different SPE techniques are tabulated and discussed .
	manualset3
215111	1	419771	7	NULL	NULL	0	NULL	SHBG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	SHBG was negatively associated with triglyceride ( r = -.21 ) and insulin ( r = -.47 ) concentrations and positively associated with HDLC concentrations ( r = .47 ) .
	manualset3
215112	2	419771	7	NULL	NULL	NULL	NULL	 triglyceride concentrations	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	SHBG was negatively associated with triglyceride ( r = -.21 ) and insulin ( r = -.47 ) concentrations and positively associated with HDLC concentrations ( r = .47 ) .
	manualset3
215113	3	419771	7	NULL	NULL	0	NULL	r = -.21	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	SHBG was negatively associated with triglyceride ( r = -.21 ) and insulin ( r = -.47 ) concentrations and positively associated with HDLC concentrations ( r = .47 ) .
	manualset3
215114	4	419771	7	NULL	NULL	NULL	NULL	insulin concentrations	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	SHBG was negatively associated with triglyceride ( r = -.21 ) and insulin ( r = -.47 ) concentrations and positively associated with HDLC concentrations ( r = .47 ) .
	manualset3
215115	5	419771	7	NULL	NULL	0	NULL	r = -.47	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	SHBG was negatively associated with triglyceride ( r = -.21 ) and insulin ( r = -.47 ) concentrations and positively associated with HDLC concentrations ( r = .47 ) .
	manualset3
215116	6	419771	7	NULL	NULL	0	NULL	HDLC concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	SHBG was negatively associated with triglyceride ( r = -.21 ) and insulin ( r = -.47 ) concentrations and positively associated with HDLC concentrations ( r = .47 ) .
	manualset3
215117	7	419771	7	NULL	NULL	0	NULL	r = .47	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	SHBG was negatively associated with triglyceride ( r = -.21 ) and insulin ( r = -.47 ) concentrations and positively associated with HDLC concentrations ( r = .47 ) .
	manualset3
215118	1	419772	7	NULL	NULL	0	NULL	Chronic administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic administration of etoposide over multiple days has proved to be an effective schedule against a variety of neoplasms .
	manualset3
215119	2	419772	7	NULL	NULL	0	NULL	etoposide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic administration of etoposide over multiple days has proved to be an effective schedule against a variety of neoplasms .
	manualset3
215120	3	419772	7	NULL	NULL	0	NULL	multiple days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic administration of etoposide over multiple days has proved to be an effective schedule against a variety of neoplasms .
	manualset3
215121	4	419772	7	NULL	NULL	0	NULL	effective schedule 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic administration of etoposide over multiple days has proved to be an effective schedule against a variety of neoplasms .
	manualset3
215122	5	419772	7	NULL	NULL	0	NULL	variety of neoplasms	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic administration of etoposide over multiple days has proved to be an effective schedule against a variety of neoplasms .
	manualset3
215123	1	419773	7	NULL	NULL	0	NULL	human SYK locus	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The human SYK locus was mapped to chromosome 9 at band q22 .
	manualset3
215124	2	419773	7	NULL	NULL	0	NULL	chromosome 9	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The human SYK locus was mapped to chromosome 9 at band q22 .
	manualset3
215125	3	419773	7	NULL	NULL	0	NULL	band q22	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The human SYK locus was mapped to chromosome 9 at band q22 .
	manualset3
215126	1	419774	7	NULL	NULL	0	NULL	Proteolytic action 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteolytic action of thrombin is required for electrical activity-dependent synapse reduction .
	manualset3
215127	2	419774	7	NULL	NULL	0	NULL	thrombin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteolytic action of thrombin is required for electrical activity-dependent synapse reduction .
	manualset3
215128	3	419774	7	NULL	NULL	0	NULL	electrical activity-dependent synapse reduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteolytic action of thrombin is required for electrical activity-dependent synapse reduction .
	manualset3
215129	1	419775	7	NULL	NULL	0	NULL	Mean serum luteinizing hormone	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean serum luteinizing hormone was higher in menstruating than in amenorrheic mothers .
	manualset3
215130	2	419775	7	NULL	NULL	0	NULL	amenorrheic mothers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean serum luteinizing hormone was higher in menstruating than in amenorrheic mothers .
	manualset3
215131	1	419776	7	NULL	NULL	0	NULL	sporadic	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although sporadic from 1965 to 1969 , a major outbreak of dengue hemorrhagic fever ( DHF ) occurred for the first time in Rangoon in 1970 .
	manualset3
215132	2	419776	7	NULL	NULL	0	NULL	1965 to 1969	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Although sporadic from 1965 to 1969 , a major outbreak of dengue hemorrhagic fever ( DHF ) occurred for the first time in Rangoon in 1970 .
	manualset3
215133	3	419776	7	NULL	NULL	0	NULL	major outbreak	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although sporadic from 1965 to 1969 , a major outbreak of dengue hemorrhagic fever ( DHF ) occurred for the first time in Rangoon in 1970 .
	manualset3
215134	4	419776	7	NULL	NULL	0	NULL	dengue hemorrhagic fever ( DHF )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Although sporadic from 1965 to 1969 , a major outbreak of dengue hemorrhagic fever ( DHF ) occurred for the first time in Rangoon in 1970 .
	manualset3
215135	5	419776	7	NULL	NULL	0	NULL	first time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Although sporadic from 1965 to 1969 , a major outbreak of dengue hemorrhagic fever ( DHF ) occurred for the first time in Rangoon in 1970 .
	manualset3
215136	6	419776	7	NULL	NULL	0	NULL	Rangoon 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Although sporadic from 1965 to 1969 , a major outbreak of dengue hemorrhagic fever ( DHF ) occurred for the first time in Rangoon in 1970 .
	manualset3
215137	7	419776	7	NULL	NULL	0	NULL	1970	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Although sporadic from 1965 to 1969 , a major outbreak of dengue hemorrhagic fever ( DHF ) occurred for the first time in Rangoon in 1970 .
	manualset3
215138	1	419777	7	NULL	NULL	0	NULL	 lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , lymphocytes of DES-exposed subjects showed maximal blastogenic response to PHA at a concentration ( 0.125 microgram/ml ) two to four times lower ( P less than 0.002 ) than controls ( 0.25 microgram/ml to 0.5 microgram/ml ) .
	manualset3
215139	2	419777	7	NULL	NULL	0	NULL	 DES-exposed subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , lymphocytes of DES-exposed subjects showed maximal blastogenic response to PHA at a concentration ( 0.125 microgram/ml ) two to four times lower ( P less than 0.002 ) than controls ( 0.25 microgram/ml to 0.5 microgram/ml ) .
	manualset3
215140	3	419777	7	NULL	NULL	0	NULL	maximal blastogenic response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , lymphocytes of DES-exposed subjects showed maximal blastogenic response to PHA at a concentration ( 0.125 microgram/ml ) two to four times lower ( P less than 0.002 ) than controls ( 0.25 microgram/ml to 0.5 microgram/ml ) .
	manualset3
215141	4	419777	7	NULL	NULL	0	NULL	PHA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , lymphocytes of DES-exposed subjects showed maximal blastogenic response to PHA at a concentration ( 0.125 microgram/ml ) two to four times lower ( P less than 0.002 ) than controls ( 0.25 microgram/ml to 0.5 microgram/ml ) .
	manualset3
215142	5	419777	7	NULL	NULL	0	NULL	 concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , lymphocytes of DES-exposed subjects showed maximal blastogenic response to PHA at a concentration ( 0.125 microgram/ml ) two to four times lower ( P less than 0.002 ) than controls ( 0.25 microgram/ml to 0.5 microgram/ml ) .
	manualset3
215143	6	419777	7	NULL	NULL	0	NULL	0.125 microgram/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , lymphocytes of DES-exposed subjects showed maximal blastogenic response to PHA at a concentration ( 0.125 microgram/ml ) two to four times lower ( P less than 0.002 ) than controls ( 0.25 microgram/ml to 0.5 microgram/ml ) .
	manualset3
215144	7	419777	7	NULL	NULL	0	NULL	two to four times	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , lymphocytes of DES-exposed subjects showed maximal blastogenic response to PHA at a concentration ( 0.125 microgram/ml ) two to four times lower ( P less than 0.002 ) than controls ( 0.25 microgram/ml to 0.5 microgram/ml ) .
	manualset3
215145	8	419777	7	NULL	NULL	0	NULL	P less than 0.002	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , lymphocytes of DES-exposed subjects showed maximal blastogenic response to PHA at a concentration ( 0.125 microgram/ml ) two to four times lower ( P less than 0.002 ) than controls ( 0.25 microgram/ml to 0.5 microgram/ml ) .
	manualset3
215146	9	419777	7	NULL	NULL	0	NULL	controls	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , lymphocytes of DES-exposed subjects showed maximal blastogenic response to PHA at a concentration ( 0.125 microgram/ml ) two to four times lower ( P less than 0.002 ) than controls ( 0.25 microgram/ml to 0.5 microgram/ml ) .
	manualset3
215147	10	419777	7	NULL	NULL	0	NULL	0.25 microgram/ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , lymphocytes of DES-exposed subjects showed maximal blastogenic response to PHA at a concentration ( 0.125 microgram/ml ) two to four times lower ( P less than 0.002 ) than controls ( 0.25 microgram/ml to 0.5 microgram/ml ) .
	manualset3
215148	11	419777	7	NULL	NULL	0	NULL	0.5 microgram/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , lymphocytes of DES-exposed subjects showed maximal blastogenic response to PHA at a concentration ( 0.125 microgram/ml ) two to four times lower ( P less than 0.002 ) than controls ( 0.25 microgram/ml to 0.5 microgram/ml ) .
	manualset3
215151	1	419778	7	NULL	NULL	0	NULL	Diploid cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Diploid cells homozygous for the bgs2-null mutation , as well as homothallic bgs2-null mutant haploids undergo meiosis normally .
	manualset3
215152	2	419778	7	NULL	NULL	0	NULL	bgs2-null mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Diploid cells homozygous for the bgs2-null mutation , as well as homothallic bgs2-null mutant haploids undergo meiosis normally .
	manualset3
215153	3	419778	7	NULL	NULL	0	NULL	homothallic bgs2-null mutant haploids	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Diploid cells homozygous for the bgs2-null mutation , as well as homothallic bgs2-null mutant haploids undergo meiosis normally .
	manualset3
215154	4	419778	7	NULL	NULL	0	NULL	meiosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Diploid cells homozygous for the bgs2-null mutation , as well as homothallic bgs2-null mutant haploids undergo meiosis normally .
	manualset3
215155	1	419779	7	NULL	NULL	NULL	NULL	novel method	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A novel method for acylation is presented , based on the formation of palmitoylchloride dispersion in aqueous acetonitrile solution , using chicken cystatin as a model protein .
	manualset3
215156	2	419779	7	NULL	NULL	0	NULL	acylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel method for acylation is presented , based on the formation of palmitoylchloride dispersion in aqueous acetonitrile solution , using chicken cystatin as a model protein .
	manualset3
215157	3	419779	7	NULL	NULL	0	NULL	formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel method for acylation is presented , based on the formation of palmitoylchloride dispersion in aqueous acetonitrile solution , using chicken cystatin as a model protein .
	manualset3
215158	4	419779	7	NULL	NULL	0	NULL	palmitoylchloride dispersion 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel method for acylation is presented , based on the formation of palmitoylchloride dispersion in aqueous acetonitrile solution , using chicken cystatin as a model protein .
	manualset3
215159	5	419779	7	NULL	NULL	0	NULL	aqueous acetonitrile solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel method for acylation is presented , based on the formation of palmitoylchloride dispersion in aqueous acetonitrile solution , using chicken cystatin as a model protein .
	manualset3
215160	6	419779	7	NULL	NULL	0	NULL	chicken cystatin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel method for acylation is presented , based on the formation of palmitoylchloride dispersion in aqueous acetonitrile solution , using chicken cystatin as a model protein .
	manualset3
215161	7	419779	7	NULL	NULL	0	NULL	model protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel method for acylation is presented , based on the formation of palmitoylchloride dispersion in aqueous acetonitrile solution , using chicken cystatin as a model protein .
	manualset3
215162	1	419780	7	NULL	NULL	0	NULL	 treatments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using these treatments and control , we performed expression profiling for 18 , 144 RefSeq transcripts on biological replicates of the complete study cohort of 113 individuals ( n ( total ) = 782 ) and combined it with genome-wide SNP-genotyping data in order to map treatment-specific cis-eQTLs ( defined as SNPs located within the gene 250 kb ) .
	manualset3
215163	2	419780	7	NULL	NULL	0	NULL	control	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using these treatments and control , we performed expression profiling for 18 , 144 RefSeq transcripts on biological replicates of the complete study cohort of 113 individuals ( n ( total ) = 782 ) and combined it with genome-wide SNP-genotyping data in order to map treatment-specific cis-eQTLs ( defined as SNPs located within the gene 250 kb ) .
	manualset3
215164	3	419780	7	NULL	NULL	0	NULL	expression profiling 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using these treatments and control , we performed expression profiling for 18 , 144 RefSeq transcripts on biological replicates of the complete study cohort of 113 individuals ( n ( total ) = 782 ) and combined it with genome-wide SNP-genotyping data in order to map treatment-specific cis-eQTLs ( defined as SNPs located within the gene 250 kb ) .
	manualset3
215165	4	419780	7	NULL	NULL	0	NULL	18 RefSeq transcripts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using these treatments and control , we performed expression profiling for 18 , 144 RefSeq transcripts on biological replicates of the complete study cohort of 113 individuals ( n ( total ) = 782 ) and combined it with genome-wide SNP-genotyping data in order to map treatment-specific cis-eQTLs ( defined as SNPs located within the gene 250 kb ) .
	manualset3
215166	5	419780	7	NULL	NULL	0	NULL	144 RefSeq transcripts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using these treatments and control , we performed expression profiling for 18 , 144 RefSeq transcripts on biological replicates of the complete study cohort of 113 individuals ( n ( total ) = 782 ) and combined it with genome-wide SNP-genotyping data in order to map treatment-specific cis-eQTLs ( defined as SNPs located within the gene 250 kb ) .
	manualset3
215167	6	419780	7	NULL	NULL	0	NULL	 biological replicates	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Using these treatments and control , we performed expression profiling for 18 , 144 RefSeq transcripts on biological replicates of the complete study cohort of 113 individuals ( n ( total ) = 782 ) and combined it with genome-wide SNP-genotyping data in order to map treatment-specific cis-eQTLs ( defined as SNPs located within the gene 250 kb ) .
	manualset3
215168	7	419780	7	NULL	NULL	0	NULL	complete study cohort	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Using these treatments and control , we performed expression profiling for 18 , 144 RefSeq transcripts on biological replicates of the complete study cohort of 113 individuals ( n ( total ) = 782 ) and combined it with genome-wide SNP-genotyping data in order to map treatment-specific cis-eQTLs ( defined as SNPs located within the gene 250 kb ) .
	manualset3
215169	8	419780	7	NULL	NULL	0	NULL	113 individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using these treatments and control , we performed expression profiling for 18 , 144 RefSeq transcripts on biological replicates of the complete study cohort of 113 individuals ( n ( total ) = 782 ) and combined it with genome-wide SNP-genotyping data in order to map treatment-specific cis-eQTLs ( defined as SNPs located within the gene 250 kb ) .
	manualset3
215170	9	419780	7	NULL	NULL	0	NULL	( n ( total ) = 782 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using these treatments and control , we performed expression profiling for 18 , 144 RefSeq transcripts on biological replicates of the complete study cohort of 113 individuals ( n ( total ) = 782 ) and combined it with genome-wide SNP-genotyping data in order to map treatment-specific cis-eQTLs ( defined as SNPs located within the gene 250 kb ) .
	manualset3
215171	10	419780	7	NULL	NULL	0	NULL	genome-wide SNP-genotyping data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Using these treatments and control , we performed expression profiling for 18 , 144 RefSeq transcripts on biological replicates of the complete study cohort of 113 individuals ( n ( total ) = 782 ) and combined it with genome-wide SNP-genotyping data in order to map treatment-specific cis-eQTLs ( defined as SNPs located within the gene 250 kb ) .
	manualset3
215172	11	419780	7	NULL	NULL	0	NULL	treatment-specific cis-eQTLs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using these treatments and control , we performed expression profiling for 18 , 144 RefSeq transcripts on biological replicates of the complete study cohort of 113 individuals ( n ( total ) = 782 ) and combined it with genome-wide SNP-genotyping data in order to map treatment-specific cis-eQTLs ( defined as SNPs located within the gene 250 kb ) .
	manualset3
215173	12	419780	7	NULL	NULL	0	NULL	SNPs	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using these treatments and control , we performed expression profiling for 18 , 144 RefSeq transcripts on biological replicates of the complete study cohort of 113 individuals ( n ( total ) = 782 ) and combined it with genome-wide SNP-genotyping data in order to map treatment-specific cis-eQTLs ( defined as SNPs located within the gene 250 kb ) .
	manualset3
215174	13	419780	7	NULL	NULL	0	NULL	gene 250 kb 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Using these treatments and control , we performed expression profiling for 18 , 144 RefSeq transcripts on biological replicates of the complete study cohort of 113 individuals ( n ( total ) = 782 ) and combined it with genome-wide SNP-genotyping data in order to map treatment-specific cis-eQTLs ( defined as SNPs located within the gene 250 kb ) .
	manualset3
215175	1	419781	7	NULL	NULL	0	NULL	common histologic type	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common histologic type of lymphoma was diffuse large cell lymphoma with 30 % of the cases having bone marrow involvement .
	manualset3
215176	2	419781	7	NULL	NULL	0	NULL	lymphoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common histologic type of lymphoma was diffuse large cell lymphoma with 30 % of the cases having bone marrow involvement .
	manualset3
215177	3	419781	7	NULL	NULL	0	NULL	large cell lymphoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common histologic type of lymphoma was diffuse large cell lymphoma with 30 % of the cases having bone marrow involvement .
	manualset3
215178	4	419781	7	NULL	NULL	0	NULL	30 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common histologic type of lymphoma was diffuse large cell lymphoma with 30 % of the cases having bone marrow involvement .
	manualset3
215179	5	419781	7	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common histologic type of lymphoma was diffuse large cell lymphoma with 30 % of the cases having bone marrow involvement .
	manualset3
215180	6	419781	7	NULL	NULL	0	NULL	bone marrow involvement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most common histologic type of lymphoma was diffuse large cell lymphoma with 30 % of the cases having bone marrow involvement .
	manualset3
215181	1	419782	7	NULL	NULL	0	NULL	reduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of the chain length from residues 1-28 to 1-27 lowered the antagonist potency while further reduction of the peptide chain led to a complete loss of inhibitory activity .
	manualset3
215182	2	419782	7	NULL	NULL	0	NULL	chain length	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of the chain length from residues 1-28 to 1-27 lowered the antagonist potency while further reduction of the peptide chain led to a complete loss of inhibitory activity .
	manualset3
215183	3	419782	7	NULL	NULL	NULL	NULL	residues 1-28	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reduction of the chain length from residues 1-28 to 1-27 lowered the antagonist potency while further reduction of the peptide chain led to a complete loss of inhibitory activity .
	manualset3
215184	4	419782	7	NULL	NULL	NULL	NULL	residues 1-27	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reduction of the chain length from residues 1-28 to 1-27 lowered the antagonist potency while further reduction of the peptide chain led to a complete loss of inhibitory activity .
	manualset3
215185	5	419782	7	NULL	NULL	0	NULL	 antagonist potency	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of the chain length from residues 1-28 to 1-27 lowered the antagonist potency while further reduction of the peptide chain led to a complete loss of inhibitory activity .
	manualset3
215186	6	419782	7	NULL	NULL	0	NULL	reduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of the chain length from residues 1-28 to 1-27 lowered the antagonist potency while further reduction of the peptide chain led to a complete loss of inhibitory activity .
	manualset3
215187	7	419782	7	NULL	NULL	0	NULL	 peptide chain	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of the chain length from residues 1-28 to 1-27 lowered the antagonist potency while further reduction of the peptide chain led to a complete loss of inhibitory activity .
	manualset3
215188	8	419782	7	NULL	NULL	0	NULL	complete loss 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of the chain length from residues 1-28 to 1-27 lowered the antagonist potency while further reduction of the peptide chain led to a complete loss of inhibitory activity .
	manualset3
215189	9	419782	7	NULL	NULL	0	NULL	inhibitory activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The reduction of the chain length from residues 1-28 to 1-27 lowered the antagonist potency while further reduction of the peptide chain led to a complete loss of inhibitory activity .
	manualset3
215190	1	419783	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to osteogenic , adipogenic , and chondrogenic differentiation , these cells were able to differentiate to endothelial cells and epithelial cells expressing podocytes markers such as nephrin , podocin , and synaptopodin .
	manualset3
215191	2	419783	7	NULL	NULL	0	NULL	osteogenic differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to osteogenic , adipogenic , and chondrogenic differentiation , these cells were able to differentiate to endothelial cells and epithelial cells expressing podocytes markers such as nephrin , podocin , and synaptopodin .
	manualset3
215192	3	419783	7	NULL	NULL	0	NULL	adipogenic differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to osteogenic , adipogenic , and chondrogenic differentiation , these cells were able to differentiate to endothelial cells and epithelial cells expressing podocytes markers such as nephrin , podocin , and synaptopodin .
	manualset3
215193	4	419783	7	NULL	NULL	0	NULL	chondrogenic differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to osteogenic , adipogenic , and chondrogenic differentiation , these cells were able to differentiate to endothelial cells and epithelial cells expressing podocytes markers such as nephrin , podocin , and synaptopodin .
	manualset3
215194	5	419783	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to osteogenic , adipogenic , and chondrogenic differentiation , these cells were able to differentiate to endothelial cells and epithelial cells expressing podocytes markers such as nephrin , podocin , and synaptopodin .
	manualset3
215195	6	419783	7	NULL	NULL	0	NULL	endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to osteogenic , adipogenic , and chondrogenic differentiation , these cells were able to differentiate to endothelial cells and epithelial cells expressing podocytes markers such as nephrin , podocin , and synaptopodin .
	manualset3
215196	7	419783	7	NULL	NULL	0	NULL	epithelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to osteogenic , adipogenic , and chondrogenic differentiation , these cells were able to differentiate to endothelial cells and epithelial cells expressing podocytes markers such as nephrin , podocin , and synaptopodin .
	manualset3
215197	8	419783	7	NULL	NULL	0	NULL	podocytes markers	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to osteogenic , adipogenic , and chondrogenic differentiation , these cells were able to differentiate to endothelial cells and epithelial cells expressing podocytes markers such as nephrin , podocin , and synaptopodin .
	manualset3
215198	9	419783	7	NULL	NULL	0	NULL	nephrin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to osteogenic , adipogenic , and chondrogenic differentiation , these cells were able to differentiate to endothelial cells and epithelial cells expressing podocytes markers such as nephrin , podocin , and synaptopodin .
	manualset3
215199	10	419783	7	NULL	NULL	0	NULL	podocin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to osteogenic , adipogenic , and chondrogenic differentiation , these cells were able to differentiate to endothelial cells and epithelial cells expressing podocytes markers such as nephrin , podocin , and synaptopodin .
	manualset3
215200	11	419783	7	NULL	NULL	0	NULL	synaptopodin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to osteogenic , adipogenic , and chondrogenic differentiation , these cells were able to differentiate to endothelial cells and epithelial cells expressing podocytes markers such as nephrin , podocin , and synaptopodin .
	manualset3
215201	1	419784	7	NULL	NULL	0	NULL	Membrane cholesterol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Membrane cholesterol protects against the changes of hemoglobin .
	manualset3
215202	2	419784	7	NULL	NULL	0	NULL	changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Membrane cholesterol protects against the changes of hemoglobin .
	manualset3
215203	3	419784	7	NULL	NULL	0	NULL	hemoglobin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Membrane cholesterol protects against the changes of hemoglobin .
	manualset3
215204	1	419785	7	NULL	NULL	0	NULL	stent placement	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Although stent placement during primary PTCA has been demonstrated to be safe and even to improve the angiographic results achieved by balloon-alone PTCA , there are few data on stent placement during rescue PTCA after failed thrombolysis .
	manualset3
215205	2	419785	7	NULL	NULL	0	NULL	primary PTCA	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Although stent placement during primary PTCA has been demonstrated to be safe and even to improve the angiographic results achieved by balloon-alone PTCA , there are few data on stent placement during rescue PTCA after failed thrombolysis .
	manualset3
215206	3	419785	7	NULL	NULL	0	NULL	angiographic results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although stent placement during primary PTCA has been demonstrated to be safe and even to improve the angiographic results achieved by balloon-alone PTCA , there are few data on stent placement during rescue PTCA after failed thrombolysis .
	manualset3
215207	4	419785	7	NULL	NULL	0	NULL	balloon-alone PTCA	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Although stent placement during primary PTCA has been demonstrated to be safe and even to improve the angiographic results achieved by balloon-alone PTCA , there are few data on stent placement during rescue PTCA after failed thrombolysis .
	manualset3
215208	5	419785	7	NULL	NULL	0	NULL	few data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Although stent placement during primary PTCA has been demonstrated to be safe and even to improve the angiographic results achieved by balloon-alone PTCA , there are few data on stent placement during rescue PTCA after failed thrombolysis .
	manualset3
215209	6	419785	7	NULL	NULL	0	NULL	stent placement	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Although stent placement during primary PTCA has been demonstrated to be safe and even to improve the angiographic results achieved by balloon-alone PTCA , there are few data on stent placement during rescue PTCA after failed thrombolysis .
	manualset3
215210	7	419785	7	NULL	NULL	0	NULL	rescue PTCA	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Although stent placement during primary PTCA has been demonstrated to be safe and even to improve the angiographic results achieved by balloon-alone PTCA , there are few data on stent placement during rescue PTCA after failed thrombolysis .
	manualset3
215211	8	419785	7	NULL	NULL	NULL	NULL	failed thrombolysis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although stent placement during primary PTCA has been demonstrated to be safe and even to improve the angiographic results achieved by balloon-alone PTCA , there are few data on stent placement during rescue PTCA after failed thrombolysis .
	manualset3
215212	1	419786	7	NULL	NULL	0	NULL	 similarities	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to these similarities , it was thought that a monoclonal antibody that inhibits the light activation of the rod outer segment GTP-binding protein , tranducin ( Gt ) , might exert some functional effect upon the G proteins that regulate the adenylate cyclase system .
	manualset3
215213	2	419786	7	NULL	NULL	0	NULL	monoclonal antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to these similarities , it was thought that a monoclonal antibody that inhibits the light activation of the rod outer segment GTP-binding protein , tranducin ( Gt ) , might exert some functional effect upon the G proteins that regulate the adenylate cyclase system .
	manualset3
215214	3	419786	7	NULL	NULL	0	NULL	 light activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to these similarities , it was thought that a monoclonal antibody that inhibits the light activation of the rod outer segment GTP-binding protein , tranducin ( Gt ) , might exert some functional effect upon the G proteins that regulate the adenylate cyclase system .
	manualset3
215215	4	419786	7	NULL	NULL	0	NULL	rod outer segment GTP-binding protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to these similarities , it was thought that a monoclonal antibody that inhibits the light activation of the rod outer segment GTP-binding protein , tranducin ( Gt ) , might exert some functional effect upon the G proteins that regulate the adenylate cyclase system .
	manualset3
215216	5	419786	7	NULL	NULL	0	NULL	tranducin ( Gt )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to these similarities , it was thought that a monoclonal antibody that inhibits the light activation of the rod outer segment GTP-binding protein , tranducin ( Gt ) , might exert some functional effect upon the G proteins that regulate the adenylate cyclase system .
	manualset3
215217	6	419786	7	NULL	NULL	0	NULL	functional effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to these similarities , it was thought that a monoclonal antibody that inhibits the light activation of the rod outer segment GTP-binding protein , tranducin ( Gt ) , might exert some functional effect upon the G proteins that regulate the adenylate cyclase system .
	manualset3
215218	7	419786	7	NULL	NULL	0	NULL	G proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to these similarities , it was thought that a monoclonal antibody that inhibits the light activation of the rod outer segment GTP-binding protein , tranducin ( Gt ) , might exert some functional effect upon the G proteins that regulate the adenylate cyclase system .
	manualset3
215219	8	419786	7	NULL	NULL	0	NULL	adenylate cyclase system	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to these similarities , it was thought that a monoclonal antibody that inhibits the light activation of the rod outer segment GTP-binding protein , tranducin ( Gt ) , might exert some functional effect upon the G proteins that regulate the adenylate cyclase system .
	manualset3
215220	1	419787	7	NULL	NULL	0	NULL	Brain uptake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Brain uptake of ( 3H ) cortisol was increased in the hypothalamus of P-gp-deficient mice compared with wild-type controls , but no differences were detected in other regions .
	manualset3
215221	2	419787	7	NULL	NULL	NULL	NULL	 (3H ) cortisol	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Brain uptake of ( 3H ) cortisol was increased in the hypothalamus of P-gp-deficient mice compared with wild-type controls , but no differences were detected in other regions .
	manualset3
215222	3	419787	7	NULL	NULL	0	NULL	 hypothalamus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Brain uptake of ( 3H ) cortisol was increased in the hypothalamus of P-gp-deficient mice compared with wild-type controls , but no differences were detected in other regions .
	manualset3
215223	4	419787	7	NULL	NULL	0	NULL	P-gp-deficient mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Brain uptake of ( 3H ) cortisol was increased in the hypothalamus of P-gp-deficient mice compared with wild-type controls , but no differences were detected in other regions .
	manualset3
215224	5	419787	7	NULL	NULL	0	NULL	wild-type controls	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Brain uptake of ( 3H ) cortisol was increased in the hypothalamus of P-gp-deficient mice compared with wild-type controls , but no differences were detected in other regions .
	manualset3
215225	6	419787	7	NULL	NULL	0	NULL	no differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Brain uptake of ( 3H ) cortisol was increased in the hypothalamus of P-gp-deficient mice compared with wild-type controls , but no differences were detected in other regions .
	manualset3
215226	7	419787	7	NULL	NULL	0	NULL	other regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Brain uptake of ( 3H ) cortisol was increased in the hypothalamus of P-gp-deficient mice compared with wild-type controls , but no differences were detected in other regions .
	manualset3
215227	1	419788	7	NULL	NULL	0	NULL	Health researchers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Health researchers , searching for a pathway to explain the adverse health outcomes associated with income inequality , as well as to understand the results of multi-level analyses that demonstrate an independent etiological role for community of residence , may find social capital an attractive notion .
	manualset3
215228	2	419788	7	NULL	NULL	0	NULL	searching	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Health researchers , searching for a pathway to explain the adverse health outcomes associated with income inequality , as well as to understand the results of multi-level analyses that demonstrate an independent etiological role for community of residence , may find social capital an attractive notion .
	manualset3
215229	3	419788	7	NULL	NULL	0	NULL	pathway	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Health researchers , searching for a pathway to explain the adverse health outcomes associated with income inequality , as well as to understand the results of multi-level analyses that demonstrate an independent etiological role for community of residence , may find social capital an attractive notion .
	manualset3
215230	4	419788	7	NULL	NULL	0	NULL	adverse health outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Health researchers , searching for a pathway to explain the adverse health outcomes associated with income inequality , as well as to understand the results of multi-level analyses that demonstrate an independent etiological role for community of residence , may find social capital an attractive notion .
	manualset3
215231	5	419788	7	NULL	NULL	0	NULL	income inequality	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Health researchers , searching for a pathway to explain the adverse health outcomes associated with income inequality , as well as to understand the results of multi-level analyses that demonstrate an independent etiological role for community of residence , may find social capital an attractive notion .
	manualset3
215232	6	419788	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Health researchers , searching for a pathway to explain the adverse health outcomes associated with income inequality , as well as to understand the results of multi-level analyses that demonstrate an independent etiological role for community of residence , may find social capital an attractive notion .
	manualset3
215233	7	419788	7	NULL	NULL	0	NULL	multi-level analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Health researchers , searching for a pathway to explain the adverse health outcomes associated with income inequality , as well as to understand the results of multi-level analyses that demonstrate an independent etiological role for community of residence , may find social capital an attractive notion .
	manualset3
215234	8	419788	7	NULL	NULL	0	NULL	 independent etiological role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Health researchers , searching for a pathway to explain the adverse health outcomes associated with income inequality , as well as to understand the results of multi-level analyses that demonstrate an independent etiological role for community of residence , may find social capital an attractive notion .
	manualset3
215235	9	419788	7	NULL	NULL	0	NULL	community	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Health researchers , searching for a pathway to explain the adverse health outcomes associated with income inequality , as well as to understand the results of multi-level analyses that demonstrate an independent etiological role for community of residence , may find social capital an attractive notion .
	manualset3
215236	10	419788	7	NULL	NULL	NULL	NULL	residence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Health researchers , searching for a pathway to explain the adverse health outcomes associated with income inequality , as well as to understand the results of multi-level analyses that demonstrate an independent etiological role for community of residence , may find social capital an attractive notion .
	manualset3
215237	11	419788	7	NULL	NULL	0	NULL	social capital 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Health researchers , searching for a pathway to explain the adverse health outcomes associated with income inequality , as well as to understand the results of multi-level analyses that demonstrate an independent etiological role for community of residence , may find social capital an attractive notion .
	manualset3
215238	12	419788	7	NULL	NULL	0	NULL	 notion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Health researchers , searching for a pathway to explain the adverse health outcomes associated with income inequality , as well as to understand the results of multi-level analyses that demonstrate an independent etiological role for community of residence , may find social capital an attractive notion .
	manualset3
215239	1	419789	7	NULL	NULL	0	NULL	 SHI heterodimer	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The SHI heterodimer and POR therefore represent a two-enzyme system that oxidizes pyruvate and produces H ( 2 ) in vitro without the need for an intermediate electron carrier .
	manualset3
215240	2	419789	7	NULL	NULL	0	NULL	POR 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The SHI heterodimer and POR therefore represent a two-enzyme system that oxidizes pyruvate and produces H ( 2 ) in vitro without the need for an intermediate electron carrier .
	manualset3
215241	3	419789	7	NULL	NULL	0	NULL	two-enzyme system	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The SHI heterodimer and POR therefore represent a two-enzyme system that oxidizes pyruvate and produces H ( 2 ) in vitro without the need for an intermediate electron carrier .
	manualset3
215242	4	419789	7	NULL	NULL	0	NULL	 pyruvate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The SHI heterodimer and POR therefore represent a two-enzyme system that oxidizes pyruvate and produces H ( 2 ) in vitro without the need for an intermediate electron carrier .
	manualset3
215243	5	419789	7	NULL	NULL	0	NULL	H ( 2 )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The SHI heterodimer and POR therefore represent a two-enzyme system that oxidizes pyruvate and produces H ( 2 ) in vitro without the need for an intermediate electron carrier .
	manualset3
215244	6	419789	7	NULL	NULL	0	NULL	need	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The SHI heterodimer and POR therefore represent a two-enzyme system that oxidizes pyruvate and produces H ( 2 ) in vitro without the need for an intermediate electron carrier .
	manualset3
215245	7	419789	7	NULL	NULL	NULL	NULL	intermediate electron carrier	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The SHI heterodimer and POR therefore represent a two-enzyme system that oxidizes pyruvate and produces H ( 2 ) in vitro without the need for an intermediate electron carrier .
	manualset3
215246	1	419790	7	NULL	NULL	0	NULL	`` Ir ( ppy ) ( 2 ) '' units	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The `` Ir ( ppy ) ( 2 ) '' units in compound 5 are noninteracting as the electronic conduit is truncated by the ethane spacer in the bpfd bridge .
	manualset3
215247	2	419790	7	NULL	NULL	0	NULL	compound 5	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The `` Ir ( ppy ) ( 2 ) '' units in compound 5 are noninteracting as the electronic conduit is truncated by the ethane spacer in the bpfd bridge .
	manualset3
215248	3	419790	7	NULL	NULL	0	NULL	noninteracting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The `` Ir ( ppy ) ( 2 ) '' units in compound 5 are noninteracting as the electronic conduit is truncated by the ethane spacer in the bpfd bridge .
	manualset3
215249	4	419790	7	NULL	NULL	0	NULL	electronic conduit	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The `` Ir ( ppy ) ( 2 ) '' units in compound 5 are noninteracting as the electronic conduit is truncated by the ethane spacer in the bpfd bridge .
	manualset3
215250	5	419790	7	NULL	NULL	0	NULL	ethane spacer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The `` Ir ( ppy ) ( 2 ) '' units in compound 5 are noninteracting as the electronic conduit is truncated by the ethane spacer in the bpfd bridge .
	manualset3
215251	6	419790	7	NULL	NULL	0	NULL	bpfd bridge 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The `` Ir ( ppy ) ( 2 ) '' units in compound 5 are noninteracting as the electronic conduit is truncated by the ethane spacer in the bpfd bridge .
	manualset3
215252	1	419791	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , a nuclear `` stethoscope '' that generates a left ventricular volume curve may soon bring this valuable resource into office practice .
	manualset3
215253	2	419791	7	NULL	NULL	0	NULL	 nuclear `` stethoscope ''	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , a nuclear `` stethoscope '' that generates a left ventricular volume curve may soon bring this valuable resource into office practice .
	manualset3
215254	3	419791	7	NULL	NULL	0	NULL	left ventricular volume curve	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , a nuclear `` stethoscope '' that generates a left ventricular volume curve may soon bring this valuable resource into office practice .
	manualset3
215255	4	419791	7	NULL	NULL	0	NULL	valuable resource	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , a nuclear `` stethoscope '' that generates a left ventricular volume curve may soon bring this valuable resource into office practice .
	manualset3
215256	5	419791	7	NULL	NULL	0	NULL	office practice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , a nuclear `` stethoscope '' that generates a left ventricular volume curve may soon bring this valuable resource into office practice .
	manualset3
215257	1	419792	7	NULL	NULL	0	NULL	trauma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The trauma of high free fall as seen at Harlem Hospital .
	manualset3
215258	2	419792	7	NULL	NULL	0	NULL	high free fall	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The trauma of high free fall as seen at Harlem Hospital .
	manualset3
215259	3	419792	7	NULL	NULL	0	NULL	Harlem Hospital 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The trauma of high free fall as seen at Harlem Hospital .
	manualset3
215260	1	419793	7	NULL	NULL	0	NULL	structurally dissimilar	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Although structurally dissimilar , both classes of molecules lead to the arrest of cell division and eventual cell death by stabilizing cellular microtubule assemblies .
	manualset3
215261	2	419793	7	NULL	NULL	0	NULL	classes of molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Although structurally dissimilar , both classes of molecules lead to the arrest of cell division and eventual cell death by stabilizing cellular microtubule assemblies .
	manualset3
215262	3	419793	7	NULL	NULL	0	NULL	arrest	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although structurally dissimilar , both classes of molecules lead to the arrest of cell division and eventual cell death by stabilizing cellular microtubule assemblies .
	manualset3
215263	4	419793	7	NULL	NULL	0	NULL	cell division	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although structurally dissimilar , both classes of molecules lead to the arrest of cell division and eventual cell death by stabilizing cellular microtubule assemblies .
	manualset3
215264	5	419793	7	NULL	NULL	0	NULL	cell death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although structurally dissimilar , both classes of molecules lead to the arrest of cell division and eventual cell death by stabilizing cellular microtubule assemblies .
	manualset3
215265	6	419793	7	NULL	NULL	0	NULL	cellular microtubule assemblies	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Although structurally dissimilar , both classes of molecules lead to the arrest of cell division and eventual cell death by stabilizing cellular microtubule assemblies .
	manualset3
215266	1	419794	7	NULL	NULL	0	NULL	Huntington 's disease ( HD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Huntington 's disease ( HD ) is an inherited , progressive neurodegenerative disorder caused by CAG repeat expansion in the gene that codes for the protein huntingtin .
	manualset3
215267	2	419794	7	NULL	NULL	0	NULL	inherited , progressive neurodegenerative disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Huntington 's disease ( HD ) is an inherited , progressive neurodegenerative disorder caused by CAG repeat expansion in the gene that codes for the protein huntingtin .
	manualset3
215268	3	419794	7	NULL	NULL	0	NULL	CAG repeat expansion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Huntington 's disease ( HD ) is an inherited , progressive neurodegenerative disorder caused by CAG repeat expansion in the gene that codes for the protein huntingtin .
	manualset3
215269	4	419794	7	NULL	NULL	0	NULL	gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Huntington 's disease ( HD ) is an inherited , progressive neurodegenerative disorder caused by CAG repeat expansion in the gene that codes for the protein huntingtin .
	manualset3
215270	5	419794	7	NULL	NULL	0	NULL	protein huntingtin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Huntington 's disease ( HD ) is an inherited , progressive neurodegenerative disorder caused by CAG repeat expansion in the gene that codes for the protein huntingtin .
	manualset3
215271	1	419795	7	NULL	NULL	NULL	NULL	activity 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The activity of efferent fibers to the pancreas , liver , and adrenal medulla is modulated by both central glucose-responsive neurons and peripheral ( gustatory , intestinal and hepatic ) glucose sensors .
	manualset3
215272	2	419795	7	NULL	NULL	0	NULL	efferent fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of efferent fibers to the pancreas , liver , and adrenal medulla is modulated by both central glucose-responsive neurons and peripheral ( gustatory , intestinal and hepatic ) glucose sensors .
	manualset3
215273	3	419795	7	NULL	NULL	0	NULL	pancreas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of efferent fibers to the pancreas , liver , and adrenal medulla is modulated by both central glucose-responsive neurons and peripheral ( gustatory , intestinal and hepatic ) glucose sensors .
	manualset3
215274	4	419795	7	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of efferent fibers to the pancreas , liver , and adrenal medulla is modulated by both central glucose-responsive neurons and peripheral ( gustatory , intestinal and hepatic ) glucose sensors .
	manualset3
215275	5	419795	7	NULL	NULL	0	NULL	adrenal medulla 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of efferent fibers to the pancreas , liver , and adrenal medulla is modulated by both central glucose-responsive neurons and peripheral ( gustatory , intestinal and hepatic ) glucose sensors .
	manualset3
215276	6	419795	7	NULL	NULL	0	NULL	central glucose-responsive neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of efferent fibers to the pancreas , liver , and adrenal medulla is modulated by both central glucose-responsive neurons and peripheral ( gustatory , intestinal and hepatic ) glucose sensors .
	manualset3
215277	7	419795	7	NULL	NULL	NULL	NULL	peripheral glucose sensors	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The activity of efferent fibers to the pancreas , liver , and adrenal medulla is modulated by both central glucose-responsive neurons and peripheral ( gustatory , intestinal and hepatic ) glucose sensors .
	manualset3
215278	8	419795	7	NULL	NULL	NULL	NULL	gustatory sensors	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The activity of efferent fibers to the pancreas , liver , and adrenal medulla is modulated by both central glucose-responsive neurons and peripheral ( gustatory , intestinal and hepatic ) glucose sensors .
	manualset3
215279	9	419795	7	NULL	NULL	0	NULL	 intestinal sensors	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of efferent fibers to the pancreas , liver , and adrenal medulla is modulated by both central glucose-responsive neurons and peripheral ( gustatory , intestinal and hepatic ) glucose sensors .
	manualset3
215280	10	419795	7	NULL	NULL	0	NULL	hepatic sensors	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The activity of efferent fibers to the pancreas , liver , and adrenal medulla is modulated by both central glucose-responsive neurons and peripheral ( gustatory , intestinal and hepatic ) glucose sensors .
	manualset3
215281	1	419796	7	NULL	NULL	0	NULL	18 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 18 patients , seven ( group 1A ) had valvular involvement and 11 ( group 1B ) had none , as determined by clinical , roentgenographic , and echocardiographic ( M-mode and 2-D ) techniques .
	manualset3
215282	2	419796	7	NULL	NULL	0	NULL	 seven	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 18 patients , seven ( group 1A ) had valvular involvement and 11 ( group 1B ) had none , as determined by clinical , roentgenographic , and echocardiographic ( M-mode and 2-D ) techniques .
	manualset3
215283	3	419796	7	NULL	NULL	0	NULL	group 1A	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 18 patients , seven ( group 1A ) had valvular involvement and 11 ( group 1B ) had none , as determined by clinical , roentgenographic , and echocardiographic ( M-mode and 2-D ) techniques .
	manualset3
215284	4	419796	7	NULL	NULL	0	NULL	 valvular involvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 18 patients , seven ( group 1A ) had valvular involvement and 11 ( group 1B ) had none , as determined by clinical , roentgenographic , and echocardiographic ( M-mode and 2-D ) techniques .
	manualset3
215285	5	419796	7	NULL	NULL	0	NULL	11	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 18 patients , seven ( group 1A ) had valvular involvement and 11 ( group 1B ) had none , as determined by clinical , roentgenographic , and echocardiographic ( M-mode and 2-D ) techniques .
	manualset3
215286	6	419796	7	NULL	NULL	0	NULL	group 1B	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 18 patients , seven ( group 1A ) had valvular involvement and 11 ( group 1B ) had none , as determined by clinical , roentgenographic , and echocardiographic ( M-mode and 2-D ) techniques .
	manualset3
215287	7	419796	7	NULL	NULL	0	NULL	 clinical techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 18 patients , seven ( group 1A ) had valvular involvement and 11 ( group 1B ) had none , as determined by clinical , roentgenographic , and echocardiographic ( M-mode and 2-D ) techniques .
	manualset3
215288	8	419796	7	NULL	NULL	0	NULL	roentgenographic techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 18 patients , seven ( group 1A ) had valvular involvement and 11 ( group 1B ) had none , as determined by clinical , roentgenographic , and echocardiographic ( M-mode and 2-D ) techniques .
	manualset3
215289	9	419796	7	NULL	NULL	0	NULL	echocardiographic ( M-mode and 2-D ) techniques 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 18 patients , seven ( group 1A ) had valvular involvement and 11 ( group 1B ) had none , as determined by clinical , roentgenographic , and echocardiographic ( M-mode and 2-D ) techniques .
	manualset3
215290	1	419797	7	NULL	NULL	0	NULL	key finding 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A key finding was insulin mRNA being detected in the underlying HepG2 cells , signifying that some of the plasmid was transported across the intestinal epithelial layer while retaining at least partial bioactivity .
	manualset3
215291	2	419797	7	NULL	NULL	0	NULL	insulin mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A key finding was insulin mRNA being detected in the underlying HepG2 cells , signifying that some of the plasmid was transported across the intestinal epithelial layer while retaining at least partial bioactivity .
	manualset3
215292	3	419797	7	NULL	NULL	0	NULL	underlying HepG2 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A key finding was insulin mRNA being detected in the underlying HepG2 cells , signifying that some of the plasmid was transported across the intestinal epithelial layer while retaining at least partial bioactivity .
	manualset3
215293	4	419797	7	NULL	NULL	0	NULL	plasmid	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A key finding was insulin mRNA being detected in the underlying HepG2 cells , signifying that some of the plasmid was transported across the intestinal epithelial layer while retaining at least partial bioactivity .
	manualset3
215294	5	419797	7	NULL	NULL	0	NULL	intestinal epithelial layer	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A key finding was insulin mRNA being detected in the underlying HepG2 cells , signifying that some of the plasmid was transported across the intestinal epithelial layer while retaining at least partial bioactivity .
	manualset3
215295	6	419797	7	NULL	NULL	NULL	NULL	partial bioactivity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A key finding was insulin mRNA being detected in the underlying HepG2 cells , signifying that some of the plasmid was transported across the intestinal epithelial layer while retaining at least partial bioactivity .
	manualset3
215296	1	419798	7	NULL	NULL	0	NULL	implications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications for nursing in this study were addressed at length in the introduction and review of the literature .
	manualset3
215297	2	419798	7	NULL	NULL	0	NULL	nursing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications for nursing in this study were addressed at length in the introduction and review of the literature .
	manualset3
215298	3	419798	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications for nursing in this study were addressed at length in the introduction and review of the literature .
	manualset3
215299	4	419798	7	NULL	NULL	0	NULL	length 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications for nursing in this study were addressed at length in the introduction and review of the literature .
	manualset3
215300	5	419798	7	NULL	NULL	0	NULL	introduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications for nursing in this study were addressed at length in the introduction and review of the literature .
	manualset3
215301	6	419798	7	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications for nursing in this study were addressed at length in the introduction and review of the literature .
	manualset3
215302	7	419798	7	NULL	NULL	0	NULL	literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The implications for nursing in this study were addressed at length in the introduction and review of the literature .
	manualset3
215303	1	419799	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , NeuroD2 is not involved in this regulatory pathway in vivo .
	manualset3
215304	2	419799	7	NULL	NULL	0	NULL	NeuroD2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , NeuroD2 is not involved in this regulatory pathway in vivo .
	manualset3
215305	3	419799	7	NULL	NULL	0	NULL	 regulatory pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , NeuroD2 is not involved in this regulatory pathway in vivo .
	manualset3
215306	1	419800	7	NULL	NULL	0	NULL	LDMC	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	LDMC and SDMC decreased during shoot elongation in spring and increased in summer , showing a significant negative correlation with SER , but were unrelated to BGR .
	manualset3
215307	2	419800	7	NULL	NULL	0	NULL	 SDMC	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	LDMC and SDMC decreased during shoot elongation in spring and increased in summer , showing a significant negative correlation with SER , but were unrelated to BGR .
	manualset3
215308	3	419800	7	NULL	NULL	0	NULL	shoot elongation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	LDMC and SDMC decreased during shoot elongation in spring and increased in summer , showing a significant negative correlation with SER , but were unrelated to BGR .
	manualset3
215309	4	419800	7	NULL	NULL	0	NULL	spring	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	LDMC and SDMC decreased during shoot elongation in spring and increased in summer , showing a significant negative correlation with SER , but were unrelated to BGR .
	manualset3
215310	5	419800	7	NULL	NULL	0	NULL	summer	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	LDMC and SDMC decreased during shoot elongation in spring and increased in summer , showing a significant negative correlation with SER , but were unrelated to BGR .
	manualset3
215311	6	419800	7	NULL	NULL	0	NULL	 negative correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	LDMC and SDMC decreased during shoot elongation in spring and increased in summer , showing a significant negative correlation with SER , but were unrelated to BGR .
	manualset3
215312	7	419800	7	NULL	NULL	0	NULL	SER	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	LDMC and SDMC decreased during shoot elongation in spring and increased in summer , showing a significant negative correlation with SER , but were unrelated to BGR .
	manualset3
215313	8	419800	7	NULL	NULL	0	NULL	BGR	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	LDMC and SDMC decreased during shoot elongation in spring and increased in summer , showing a significant negative correlation with SER , but were unrelated to BGR .
	manualset3
215314	1	419801	7	NULL	NULL	0	NULL	adenovirus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , when adenovirus encoding the anti-human MHCI intrabody was used to transduce primary human keratinocytes , a marked reduction of surface MHCI expression was observed .
	manualset3
215315	2	419801	7	NULL	NULL	0	NULL	anti-human MHCI intrabody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , when adenovirus encoding the anti-human MHCI intrabody was used to transduce primary human keratinocytes , a marked reduction of surface MHCI expression was observed .
	manualset3
215316	3	419801	7	NULL	NULL	0	NULL	primary human keratinocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , when adenovirus encoding the anti-human MHCI intrabody was used to transduce primary human keratinocytes , a marked reduction of surface MHCI expression was observed .
	manualset3
215317	4	419801	7	NULL	NULL	0	NULL	marked reduction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , when adenovirus encoding the anti-human MHCI intrabody was used to transduce primary human keratinocytes , a marked reduction of surface MHCI expression was observed .
	manualset3
215318	5	419801	7	NULL	NULL	0	NULL	surface MHCI expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , when adenovirus encoding the anti-human MHCI intrabody was used to transduce primary human keratinocytes , a marked reduction of surface MHCI expression was observed .
	manualset3
215319	1	419802	7	NULL	NULL	0	NULL	Twelve glial brain tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve glial brain tumors were analyzed , and only 1 case with amplification of the erbB1 oncogene was found .
	manualset3
215320	2	419802	7	NULL	NULL	0	NULL	1 case	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve glial brain tumors were analyzed , and only 1 case with amplification of the erbB1 oncogene was found .
	manualset3
215321	3	419802	7	NULL	NULL	0	NULL	amplification	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve glial brain tumors were analyzed , and only 1 case with amplification of the erbB1 oncogene was found .
	manualset3
215322	4	419802	7	NULL	NULL	0	NULL	erbB1 oncogene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve glial brain tumors were analyzed , and only 1 case with amplification of the erbB1 oncogene was found .
	manualset3
215323	1	419803	7	NULL	NULL	0	NULL	therapeutic strategy	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Our therapeutic strategy , based on thresholds of intervention favors the therapeutic slowness and strengthens negatively the metabolic memory .
	manualset3
215324	2	419803	7	NULL	NULL	0	NULL	 thresholds	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our therapeutic strategy , based on thresholds of intervention favors the therapeutic slowness and strengthens negatively the metabolic memory .
	manualset3
215325	3	419803	7	NULL	NULL	0	NULL	 intervention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our therapeutic strategy , based on thresholds of intervention favors the therapeutic slowness and strengthens negatively the metabolic memory .
	manualset3
215326	4	419803	7	NULL	NULL	0	NULL	therapeutic slowness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our therapeutic strategy , based on thresholds of intervention favors the therapeutic slowness and strengthens negatively the metabolic memory .
	manualset3
215327	5	419803	7	NULL	NULL	0	NULL	metabolic memory	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our therapeutic strategy , based on thresholds of intervention favors the therapeutic slowness and strengthens negatively the metabolic memory .
	manualset3
215328	1	419804	7	NULL	NULL	0	NULL	Several populations 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Several populations of antibodies are present in myasthenia gravis according to an idiotype-anti-idiotype process , reflecting the complexity of immune reactions .
	manualset3
215329	2	419804	7	NULL	NULL	0	NULL	antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Several populations of antibodies are present in myasthenia gravis according to an idiotype-anti-idiotype process , reflecting the complexity of immune reactions .
	manualset3
215330	3	419804	7	NULL	NULL	0	NULL	myasthenia gravis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Several populations of antibodies are present in myasthenia gravis according to an idiotype-anti-idiotype process , reflecting the complexity of immune reactions .
	manualset3
215331	4	419804	7	NULL	NULL	0	NULL	idiotype-anti-idiotype process	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several populations of antibodies are present in myasthenia gravis according to an idiotype-anti-idiotype process , reflecting the complexity of immune reactions .
	manualset3
215332	5	419804	7	NULL	NULL	0	NULL	complexity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several populations of antibodies are present in myasthenia gravis according to an idiotype-anti-idiotype process , reflecting the complexity of immune reactions .
	manualset3
215334	6	419804	7	NULL	NULL	NULL	NULL	immune reactions	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Several populations of antibodies are present in myasthenia gravis according to an idiotype-anti-idiotype process , reflecting the complexity of immune reactions .
	manualset3
215335	1	419805	7	NULL	NULL	0	NULL	reason	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason , patients of reproductive age with this pathology are referred for gynecology consultation .
	manualset3
215336	2	419805	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason , patients of reproductive age with this pathology are referred for gynecology consultation .
	manualset3
215337	3	419805	7	NULL	NULL	0	NULL	reproductive age	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason , patients of reproductive age with this pathology are referred for gynecology consultation .
	manualset3
215338	4	419805	7	NULL	NULL	0	NULL	pathology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason , patients of reproductive age with this pathology are referred for gynecology consultation .
	manualset3
215339	5	419805	7	NULL	NULL	0	NULL	gynecology consultation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason , patients of reproductive age with this pathology are referred for gynecology consultation .
	manualset3
215340	1	419806	7	NULL	NULL	0	NULL	teen parenthood	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although teen parenthood has been predominantly looked at with a focus on potential adverse physical , emotional , and socioeconomic outcomes for the mother and child ; a growing body of literature has documented the strengths and resiliency of young parents .
	manualset3
215341	2	419806	7	NULL	NULL	0	NULL	focus	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although teen parenthood has been predominantly looked at with a focus on potential adverse physical , emotional , and socioeconomic outcomes for the mother and child ; a growing body of literature has documented the strengths and resiliency of young parents .
	manualset3
215342	3	419806	7	NULL	NULL	NULL	NULL	physical outcome	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although teen parenthood has been predominantly looked at with a focus on potential adverse physical , emotional , and socioeconomic outcomes for the mother and child ; a growing body of literature has documented the strengths and resiliency of young parents .
	manualset3
215343	4	419806	7	NULL	NULL	0	NULL	emotional outcome	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although teen parenthood has been predominantly looked at with a focus on potential adverse physical , emotional , and socioeconomic outcomes for the mother and child ; a growing body of literature has documented the strengths and resiliency of young parents .
	manualset3
215344	5	419806	7	NULL	NULL	0	NULL	socioeconomic outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although teen parenthood has been predominantly looked at with a focus on potential adverse physical , emotional , and socioeconomic outcomes for the mother and child ; a growing body of literature has documented the strengths and resiliency of young parents .
	manualset3
215345	6	419806	7	NULL	NULL	0	NULL	mother	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Although teen parenthood has been predominantly looked at with a focus on potential adverse physical , emotional , and socioeconomic outcomes for the mother and child ; a growing body of literature has documented the strengths and resiliency of young parents .
	manualset3
215346	7	419806	7	NULL	NULL	0	NULL	child	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Although teen parenthood has been predominantly looked at with a focus on potential adverse physical , emotional , and socioeconomic outcomes for the mother and child ; a growing body of literature has documented the strengths and resiliency of young parents .
	manualset3
215347	8	419806	7	NULL	NULL	NULL	NULL	growing body of literature	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although teen parenthood has been predominantly looked at with a focus on potential adverse physical , emotional , and socioeconomic outcomes for the mother and child ; a growing body of literature has documented the strengths and resiliency of young parents .
	manualset3
215349	10	419806	7	NULL	NULL	0	NULL	strengths	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although teen parenthood has been predominantly looked at with a focus on potential adverse physical , emotional , and socioeconomic outcomes for the mother and child ; a growing body of literature has documented the strengths and resiliency of young parents .
	manualset3
215350	11	419806	7	NULL	NULL	0	NULL	resiliency	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although teen parenthood has been predominantly looked at with a focus on potential adverse physical , emotional , and socioeconomic outcomes for the mother and child ; a growing body of literature has documented the strengths and resiliency of young parents .
	manualset3
215351	12	419806	7	NULL	NULL	0	NULL	young parents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although teen parenthood has been predominantly looked at with a focus on potential adverse physical , emotional , and socioeconomic outcomes for the mother and child ; a growing body of literature has documented the strengths and resiliency of young parents .
	manualset3
215352	1	419807	7	NULL	NULL	0	NULL	Adipocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Adipocytes express two types of amine oxidases : the cell surface semicarbazide-sensitive amine oxidase ( SSAO ) and the mitochondrial monoamine oxidase ( MAO ) .
	manualset3
215353	2	419807	7	NULL	NULL	0	NULL	two types	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Adipocytes express two types of amine oxidases : the cell surface semicarbazide-sensitive amine oxidase ( SSAO ) and the mitochondrial monoamine oxidase ( MAO ) .
	manualset3
215354	3	419807	7	NULL	NULL	0	NULL	amine oxidases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Adipocytes express two types of amine oxidases : the cell surface semicarbazide-sensitive amine oxidase ( SSAO ) and the mitochondrial monoamine oxidase ( MAO ) .
	manualset3
215355	4	419807	7	NULL	NULL	0	NULL	cell surface semicarbazide-sensitive amine oxidase ( SSAO )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Adipocytes express two types of amine oxidases : the cell surface semicarbazide-sensitive amine oxidase ( SSAO ) and the mitochondrial monoamine oxidase ( MAO ) .
	manualset3
215356	5	419807	7	NULL	NULL	0	NULL	mitochondrial monoamine oxidase ( MAO )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Adipocytes express two types of amine oxidases : the cell surface semicarbazide-sensitive amine oxidase ( SSAO ) and the mitochondrial monoamine oxidase ( MAO ) .
	manualset3
215357	1	419808	7	NULL	NULL	0	NULL	Patterns 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patterns of acid-base changes during surgical convalescence .
	manualset3
215358	2	419808	7	NULL	NULL	0	NULL	acid-base changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patterns of acid-base changes during surgical convalescence .
	manualset3
215359	3	419808	7	NULL	NULL	0	NULL	surgical convalescence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patterns of acid-base changes during surgical convalescence .
	manualset3
215360	1	419809	7	NULL	NULL	0	NULL	 data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data reveal a novel function of ASAP in centrosome integrity .
	manualset3
215361	2	419809	7	NULL	NULL	0	NULL	novel function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data reveal a novel function of ASAP in centrosome integrity .
	manualset3
215362	3	419809	7	NULL	NULL	0	NULL	ASAP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data reveal a novel function of ASAP in centrosome integrity .
	manualset3
215363	4	419809	7	NULL	NULL	0	NULL	centrosome integrity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data reveal a novel function of ASAP in centrosome integrity .
	manualset3
215364	1	419810	7	NULL	NULL	0	NULL	GPI-anchored proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	GPI-anchored proteins with diverse functions as well as caveolin may be recovered in a membrane fraction insoluble in cold non-ionic detergent .
	manualset3
215365	2	419810	7	NULL	NULL	0	NULL	diverse functions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GPI-anchored proteins with diverse functions as well as caveolin may be recovered in a membrane fraction insoluble in cold non-ionic detergent .
	manualset3
215366	3	419810	7	NULL	NULL	0	NULL	caveolin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	GPI-anchored proteins with diverse functions as well as caveolin may be recovered in a membrane fraction insoluble in cold non-ionic detergent .
	manualset3
215367	4	419810	7	NULL	NULL	0	NULL	membrane fraction	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	GPI-anchored proteins with diverse functions as well as caveolin may be recovered in a membrane fraction insoluble in cold non-ionic detergent .
	manualset3
215368	5	419810	7	NULL	NULL	0	NULL	cold non-ionic detergent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	GPI-anchored proteins with diverse functions as well as caveolin may be recovered in a membrane fraction insoluble in cold non-ionic detergent .
	manualset3
215369	1	419811	7	NULL	NULL	0	NULL	two enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The two enzymes differed from each other on peptide mapping and in their heat-stabilities ; with respect to the latter the dihydrodiol dehydrogenase and 3 alpha-hydroxysteroid dehydrogenase activities of the respective enzymes were similarly inactivated .
	manualset3
215370	2	419811	7	NULL	NULL	0	NULL	peptide mapping	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The two enzymes differed from each other on peptide mapping and in their heat-stabilities ; with respect to the latter the dihydrodiol dehydrogenase and 3 alpha-hydroxysteroid dehydrogenase activities of the respective enzymes were similarly inactivated .
	manualset3
215371	3	419811	7	NULL	NULL	0	NULL	 heat-stabilities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The two enzymes differed from each other on peptide mapping and in their heat-stabilities ; with respect to the latter the dihydrodiol dehydrogenase and 3 alpha-hydroxysteroid dehydrogenase activities of the respective enzymes were similarly inactivated .
	manualset3
215372	4	419811	7	NULL	NULL	0	NULL	dihydrodiol dehydrogenase activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The two enzymes differed from each other on peptide mapping and in their heat-stabilities ; with respect to the latter the dihydrodiol dehydrogenase and 3 alpha-hydroxysteroid dehydrogenase activities of the respective enzymes were similarly inactivated .
	manualset3
215373	5	419811	7	NULL	NULL	0	NULL	3 alpha-hydroxysteroid dehydrogenase activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The two enzymes differed from each other on peptide mapping and in their heat-stabilities ; with respect to the latter the dihydrodiol dehydrogenase and 3 alpha-hydroxysteroid dehydrogenase activities of the respective enzymes were similarly inactivated .
	manualset3
215374	6	419811	7	NULL	NULL	0	NULL	enzymes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The two enzymes differed from each other on peptide mapping and in their heat-stabilities ; with respect to the latter the dihydrodiol dehydrogenase and 3 alpha-hydroxysteroid dehydrogenase activities of the respective enzymes were similarly inactivated .
	manualset3
215375	1	419812	7	NULL	NULL	0	NULL	phosphatase activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The phosphatase activity is predominantly soluble .
	manualset3
215376	2	419812	7	NULL	NULL	0	NULL	soluble	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The phosphatase activity is predominantly soluble .
	manualset3
215377	1	419813	7	NULL	NULL	0	NULL	Sleep quality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep quality , feeling rested at school and less distinct bedtimes were clearly related to school functioning .
	manualset3
215378	2	419813	7	NULL	NULL	0	NULL	feeling rested at school	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep quality , feeling rested at school and less distinct bedtimes were clearly related to school functioning .
	manualset3
215379	3	419813	7	NULL	NULL	0	NULL	less distinct bedtimes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep quality , feeling rested at school and less distinct bedtimes were clearly related to school functioning .
	manualset3
215380	4	419813	7	NULL	NULL	0	NULL	school functioning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep quality , feeling rested at school and less distinct bedtimes were clearly related to school functioning .
	manualset3
215381	1	419814	7	NULL	NULL	0	NULL	Rotational deformity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Rotational deformity was not observed in two cases .
	manualset3
215382	2	419814	7	NULL	NULL	0	NULL	two cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Rotational deformity was not observed in two cases .
	manualset3
215383	1	419815	7	NULL	NULL	0	NULL	telemedicine	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Although telemedicine clearly has a wide range of potential benefits , it also has some disadvantages .
	manualset3
215384	2	419815	7	NULL	NULL	0	NULL	wide range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although telemedicine clearly has a wide range of potential benefits , it also has some disadvantages .
	manualset3
215385	3	419815	7	NULL	NULL	0	NULL	potential benefits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although telemedicine clearly has a wide range of potential benefits , it also has some disadvantages .
	manualset3
215386	4	419815	7	NULL	NULL	0	NULL	 disadvantages	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although telemedicine clearly has a wide range of potential benefits , it also has some disadvantages .
	manualset3
215387	1	419816	7	NULL	NULL	0	NULL	 inhibitory effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory effect on adherence is also observed in the urine after oral administration of 400 mg of nitroxoline .
	manualset3
215388	2	419816	7	NULL	NULL	0	NULL	adherence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory effect on adherence is also observed in the urine after oral administration of 400 mg of nitroxoline .
	manualset3
215389	3	419816	7	NULL	NULL	0	NULL	urine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory effect on adherence is also observed in the urine after oral administration of 400 mg of nitroxoline .
	manualset3
215390	4	419816	7	NULL	NULL	0	NULL	oral administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory effect on adherence is also observed in the urine after oral administration of 400 mg of nitroxoline .
	manualset3
215391	5	419816	7	NULL	NULL	0	NULL	400 mg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory effect on adherence is also observed in the urine after oral administration of 400 mg of nitroxoline .
	manualset3
215392	6	419816	7	NULL	NULL	0	NULL	nitroxoline	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory effect on adherence is also observed in the urine after oral administration of 400 mg of nitroxoline .
	manualset3
215393	1	419817	7	NULL	NULL	0	NULL	Adiponectin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Adiponectin , derived mainly from white adipose tissue , regulates glucose and fatty acid metabolism and has anti-inflammatory and anti-atherosclerotic properties .
	manualset3
215394	2	419817	7	NULL	NULL	0	NULL	white adipose tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Adiponectin , derived mainly from white adipose tissue , regulates glucose and fatty acid metabolism and has anti-inflammatory and anti-atherosclerotic properties .
	manualset3
215395	3	419817	7	NULL	NULL	0	NULL	glucose metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Adiponectin , derived mainly from white adipose tissue , regulates glucose and fatty acid metabolism and has anti-inflammatory and anti-atherosclerotic properties .
	manualset3
215396	4	419817	7	NULL	NULL	0	NULL	fatty acid metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Adiponectin , derived mainly from white adipose tissue , regulates glucose and fatty acid metabolism and has anti-inflammatory and anti-atherosclerotic properties .
	manualset3
215397	5	419817	7	NULL	NULL	0	NULL	anti-inflammatory properties	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Adiponectin , derived mainly from white adipose tissue , regulates glucose and fatty acid metabolism and has anti-inflammatory and anti-atherosclerotic properties .
	manualset3
215398	6	419817	7	NULL	NULL	0	NULL	anti-atherosclerotic properties	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Adiponectin , derived mainly from white adipose tissue , regulates glucose and fatty acid metabolism and has anti-inflammatory and anti-atherosclerotic properties .
	manualset3
215399	1	419818	7	NULL	NULL	0	NULL	Interaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction between acetylcholine and sotalol ( MJ-1999 ) in adrenal medulla .
	manualset3
215400	2	419818	7	NULL	NULL	0	NULL	acetylcholine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction between acetylcholine and sotalol ( MJ-1999 ) in adrenal medulla .
	manualset3
215401	3	419818	7	NULL	NULL	0	NULL	sotalol ( MJ-1999 )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction between acetylcholine and sotalol ( MJ-1999 ) in adrenal medulla .
	manualset3
215402	4	419818	7	NULL	NULL	0	NULL	adrenal medulla	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Interaction between acetylcholine and sotalol ( MJ-1999 ) in adrenal medulla .
	manualset3
215403	1	419819	7	NULL	NULL	0	NULL	Experimental construction 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Experimental construction of a model for transplantation of the kidney into the pelvis ) .
	manualset3
215404	2	419819	7	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Experimental construction of a model for transplantation of the kidney into the pelvis ) .
	manualset3
215405	3	419819	7	NULL	NULL	0	NULL	transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Experimental construction of a model for transplantation of the kidney into the pelvis ) .
	manualset3
215406	4	419819	7	NULL	NULL	0	NULL	kidney	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Experimental construction of a model for transplantation of the kidney into the pelvis ) .
	manualset3
215407	5	419819	7	NULL	NULL	0	NULL	 pelvis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Experimental construction of a model for transplantation of the kidney into the pelvis ) .
	manualset3
215408	1	419820	7	NULL	NULL	0	NULL	Inhalation drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Inhalation drugs in asthma ) .
	manualset3
215409	2	419820	7	NULL	NULL	0	NULL	asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Inhalation drugs in asthma ) .
	manualset3
215410	1	419821	7	NULL	NULL	0	NULL	MMR	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MMR recognizes and repairs DNA mismatches and small insertion/deletion loops .
	manualset3
215411	2	419821	7	NULL	NULL	NULL	NULL	 DNA mismatches	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	MMR recognizes and repairs DNA mismatches and small insertion/deletion loops .
	manualset3
215412	3	419821	7	NULL	NULL	0	NULL	small insertion/deletion loops	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	MMR recognizes and repairs DNA mismatches and small insertion/deletion loops .
	manualset3
215413	1	419822	7	NULL	NULL	0	NULL	Singlet oxygen formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Singlet oxygen formation by a peroxidase , H2O2 and halide system .
	manualset3
215414	2	419822	7	NULL	NULL	0	NULL	peroxidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Singlet oxygen formation by a peroxidase , H2O2 and halide system .
	manualset3
215415	3	419822	7	NULL	NULL	0	NULL	H2O2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Singlet oxygen formation by a peroxidase , H2O2 and halide system .
	manualset3
215416	4	419822	7	NULL	NULL	0	NULL	halide system	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Singlet oxygen formation by a peroxidase , H2O2 and halide system .
	manualset3
215417	1	419823	7	NULL	NULL	0	NULL	Eight patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Eight patients died 5-352 days ( median 26 ) after filter insertion , without relation to the procedure .
	manualset3
215418	2	419823	7	NULL	NULL	0	NULL	 5-352 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Eight patients died 5-352 days ( median 26 ) after filter insertion , without relation to the procedure .
	manualset3
215419	3	419823	7	NULL	NULL	0	NULL	median 26	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Eight patients died 5-352 days ( median 26 ) after filter insertion , without relation to the procedure .
	manualset3
215420	4	419823	7	NULL	NULL	0	NULL	filter insertion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Eight patients died 5-352 days ( median 26 ) after filter insertion , without relation to the procedure .
	manualset3
215421	5	419823	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Eight patients died 5-352 days ( median 26 ) after filter insertion , without relation to the procedure .
	manualset3
215422	6	419823	7	NULL	NULL	0	NULL	procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Eight patients died 5-352 days ( median 26 ) after filter insertion , without relation to the procedure .
	manualset3
215423	1	419824	7	NULL	NULL	0	NULL	1978 Presidential Address	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1978 Presidential Address of the Southern Surgical Association is dedicated to the wives of the members , past and present , in acknowledgment and appreciation of the enduring contribution that they have made to the quality and character of this association .
	manualset3
215424	2	419824	7	NULL	NULL	0	NULL	Southern Surgical Association	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1978 Presidential Address of the Southern Surgical Association is dedicated to the wives of the members , past and present , in acknowledgment and appreciation of the enduring contribution that they have made to the quality and character of this association .
	manualset3
215425	3	419824	7	NULL	NULL	0	NULL	wives of the members	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1978 Presidential Address of the Southern Surgical Association is dedicated to the wives of the members , past and present , in acknowledgment and appreciation of the enduring contribution that they have made to the quality and character of this association .
	manualset3
215426	4	419824	7	NULL	NULL	0	NULL	acknowledgment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1978 Presidential Address of the Southern Surgical Association is dedicated to the wives of the members , past and present , in acknowledgment and appreciation of the enduring contribution that they have made to the quality and character of this association .
	manualset3
215427	5	419824	7	NULL	NULL	0	NULL	appreciation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1978 Presidential Address of the Southern Surgical Association is dedicated to the wives of the members , past and present , in acknowledgment and appreciation of the enduring contribution that they have made to the quality and character of this association .
	manualset3
215428	6	419824	7	NULL	NULL	0	NULL	 enduring contribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1978 Presidential Address of the Southern Surgical Association is dedicated to the wives of the members , past and present , in acknowledgment and appreciation of the enduring contribution that they have made to the quality and character of this association .
	manualset3
215429	7	419824	7	NULL	NULL	0	NULL	 quality 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1978 Presidential Address of the Southern Surgical Association is dedicated to the wives of the members , past and present , in acknowledgment and appreciation of the enduring contribution that they have made to the quality and character of this association .
	manualset3
215430	8	419824	7	NULL	NULL	0	NULL	character	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1978 Presidential Address of the Southern Surgical Association is dedicated to the wives of the members , past and present , in acknowledgment and appreciation of the enduring contribution that they have made to the quality and character of this association .
	manualset3
215431	9	419824	7	NULL	NULL	0	NULL	association	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The 1978 Presidential Address of the Southern Surgical Association is dedicated to the wives of the members , past and present , in acknowledgment and appreciation of the enduring contribution that they have made to the quality and character of this association .
	manualset3
215432	1	419825	7	NULL	NULL	0	NULL	Method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Method of compression arthrodesis of the shoulder joint ) .
	manualset3
215433	2	419825	7	NULL	NULL	0	NULL	compression arthrodesis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Method of compression arthrodesis of the shoulder joint ) .
	manualset3
215434	3	419825	7	NULL	NULL	0	NULL	 shoulder joint 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Method of compression arthrodesis of the shoulder joint ) .
	manualset3
215435	1	419826	7	NULL	NULL	0	NULL	Continuous recording	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuous recording of O 2 content in coronary sinus blood of conscious dogs .
	manualset3
215436	2	419826	7	NULL	NULL	0	NULL	O 2 content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuous recording of O 2 content in coronary sinus blood of conscious dogs .
	manualset3
215437	3	419826	7	NULL	NULL	0	NULL	 coronary sinus blood 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuous recording of O 2 content in coronary sinus blood of conscious dogs .
	manualset3
215438	4	419826	7	NULL	NULL	0	NULL	conscious dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuous recording of O 2 content in coronary sinus blood of conscious dogs .
	manualset3
215439	1	419827	7	NULL	NULL	0	NULL	active site structure	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The active site structure and the computational docking results suggested that probable substrates would likely include phosphorylated sugar lactones .
	manualset3
215440	2	419827	7	NULL	NULL	0	NULL	computational docking results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The active site structure and the computational docking results suggested that probable substrates would likely include phosphorylated sugar lactones .
	manualset3
215441	3	419827	7	NULL	NULL	NULL	NULL	 substrates	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The active site structure and the computational docking results suggested that probable substrates would likely include phosphorylated sugar lactones .
	manualset3
215442	4	419827	7	NULL	NULL	0	NULL	phosphorylated sugar lactones	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The active site structure and the computational docking results suggested that probable substrates would likely include phosphorylated sugar lactones .
	manualset3
215443	1	419828	7	NULL	NULL	0	NULL	Evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Evaluation of the catabolic and anticatabolic effects of adrenal and sex steroid hormones by the relation between the serum calcium level and the densitogram of the vertebrae ) .
	manualset3
215444	2	419828	7	NULL	NULL	0	NULL	catabolic effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Evaluation of the catabolic and anticatabolic effects of adrenal and sex steroid hormones by the relation between the serum calcium level and the densitogram of the vertebrae ) .
	manualset3
215445	3	419828	7	NULL	NULL	0	NULL	anticatabolic effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Evaluation of the catabolic and anticatabolic effects of adrenal and sex steroid hormones by the relation between the serum calcium level and the densitogram of the vertebrae ) .
	manualset3
215446	4	419828	7	NULL	NULL	0	NULL	adrenal hormones	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Evaluation of the catabolic and anticatabolic effects of adrenal and sex steroid hormones by the relation between the serum calcium level and the densitogram of the vertebrae ) .
	manualset3
215447	5	419828	7	NULL	NULL	0	NULL	sex steroid hormones	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Evaluation of the catabolic and anticatabolic effects of adrenal and sex steroid hormones by the relation between the serum calcium level and the densitogram of the vertebrae ) .
	manualset3
215448	6	419828	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	( Evaluation of the catabolic and anticatabolic effects of adrenal and sex steroid hormones by the relation between the serum calcium level and the densitogram of the vertebrae ) .
	manualset3
215449	7	419828	7	NULL	NULL	0	NULL	serum calcium level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Evaluation of the catabolic and anticatabolic effects of adrenal and sex steroid hormones by the relation between the serum calcium level and the densitogram of the vertebrae ) .
	manualset3
215450	8	419828	7	NULL	NULL	0	NULL	densitogram	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Evaluation of the catabolic and anticatabolic effects of adrenal and sex steroid hormones by the relation between the serum calcium level and the densitogram of the vertebrae ) .
	manualset3
215451	9	419828	7	NULL	NULL	0	NULL	vertebrae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Evaluation of the catabolic and anticatabolic effects of adrenal and sex steroid hormones by the relation between the serum calcium level and the densitogram of the vertebrae ) .
	manualset3
215452	1	419829	7	NULL	NULL	0	NULL	 frequency 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of mutations according to phenotype was 5.7 % ( 20/352 ) in fvFTD , 17.9 % ( 19/106 ) in familial forms , 4.4 % in PPA ( 3/68 ) , 3.3 % in CBDS ( 1/30 ) .
	manualset3
215453	2	419829	7	NULL	NULL	0	NULL	mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of mutations according to phenotype was 5.7 % ( 20/352 ) in fvFTD , 17.9 % ( 19/106 ) in familial forms , 4.4 % in PPA ( 3/68 ) , 3.3 % in CBDS ( 1/30 ) .
	manualset3
215454	3	419829	7	NULL	NULL	0	NULL	phenotype	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of mutations according to phenotype was 5.7 % ( 20/352 ) in fvFTD , 17.9 % ( 19/106 ) in familial forms , 4.4 % in PPA ( 3/68 ) , 3.3 % in CBDS ( 1/30 ) .
	manualset3
215455	4	419829	7	NULL	NULL	0	NULL	 5.7 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of mutations according to phenotype was 5.7 % ( 20/352 ) in fvFTD , 17.9 % ( 19/106 ) in familial forms , 4.4 % in PPA ( 3/68 ) , 3.3 % in CBDS ( 1/30 ) .
	manualset3
215456	5	419829	7	NULL	NULL	0	NULL	20/352	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of mutations according to phenotype was 5.7 % ( 20/352 ) in fvFTD , 17.9 % ( 19/106 ) in familial forms , 4.4 % in PPA ( 3/68 ) , 3.3 % in CBDS ( 1/30 ) .
	manualset3
215457	6	419829	7	NULL	NULL	0	NULL	fvFTD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of mutations according to phenotype was 5.7 % ( 20/352 ) in fvFTD , 17.9 % ( 19/106 ) in familial forms , 4.4 % in PPA ( 3/68 ) , 3.3 % in CBDS ( 1/30 ) .
	manualset3
215458	7	419829	7	NULL	NULL	0	NULL	17.9 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of mutations according to phenotype was 5.7 % ( 20/352 ) in fvFTD , 17.9 % ( 19/106 ) in familial forms , 4.4 % in PPA ( 3/68 ) , 3.3 % in CBDS ( 1/30 ) .
	manualset3
215459	8	419829	7	NULL	NULL	0	NULL	19/106 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of mutations according to phenotype was 5.7 % ( 20/352 ) in fvFTD , 17.9 % ( 19/106 ) in familial forms , 4.4 % in PPA ( 3/68 ) , 3.3 % in CBDS ( 1/30 ) .
	manualset3
215460	9	419829	7	NULL	NULL	0	NULL	familial forms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of mutations according to phenotype was 5.7 % ( 20/352 ) in fvFTD , 17.9 % ( 19/106 ) in familial forms , 4.4 % in PPA ( 3/68 ) , 3.3 % in CBDS ( 1/30 ) .
	manualset3
215461	10	419829	7	NULL	NULL	0	NULL	4.4 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of mutations according to phenotype was 5.7 % ( 20/352 ) in fvFTD , 17.9 % ( 19/106 ) in familial forms , 4.4 % in PPA ( 3/68 ) , 3.3 % in CBDS ( 1/30 ) .
	manualset3
215462	11	419829	7	NULL	NULL	0	NULL	 PPA	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of mutations according to phenotype was 5.7 % ( 20/352 ) in fvFTD , 17.9 % ( 19/106 ) in familial forms , 4.4 % in PPA ( 3/68 ) , 3.3 % in CBDS ( 1/30 ) .
	manualset3
215463	12	419829	7	NULL	NULL	0	NULL	3/68	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of mutations according to phenotype was 5.7 % ( 20/352 ) in fvFTD , 17.9 % ( 19/106 ) in familial forms , 4.4 % in PPA ( 3/68 ) , 3.3 % in CBDS ( 1/30 ) .
	manualset3
215464	13	419829	7	NULL	NULL	0	NULL	3.3 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of mutations according to phenotype was 5.7 % ( 20/352 ) in fvFTD , 17.9 % ( 19/106 ) in familial forms , 4.4 % in PPA ( 3/68 ) , 3.3 % in CBDS ( 1/30 ) .
	manualset3
215465	14	419829	7	NULL	NULL	0	NULL	CBDS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of mutations according to phenotype was 5.7 % ( 20/352 ) in fvFTD , 17.9 % ( 19/106 ) in familial forms , 4.4 % in PPA ( 3/68 ) , 3.3 % in CBDS ( 1/30 ) .
	manualset3
215466	15	419829	7	NULL	NULL	0	NULL	1/30	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of mutations according to phenotype was 5.7 % ( 20/352 ) in fvFTD , 17.9 % ( 19/106 ) in familial forms , 4.4 % in PPA ( 3/68 ) , 3.3 % in CBDS ( 1/30 ) .
	manualset3
215467	1	419830	7	NULL	NULL	0	NULL	HRM scores	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	HRM scores were also compared to sequenced-based measures of HIV diversity ; higher HRM scores were associated with higher genetic diversity ( p & lt ; 0.001 ) , complexity ( p = 0.009 ) , and Shannon entropy ( p = 0.022 ) , but not with length variation ( p = 0.111 ) .
	manualset3
215468	2	419830	7	NULL	NULL	0	NULL	sequenced-based measures 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	HRM scores were also compared to sequenced-based measures of HIV diversity ; higher HRM scores were associated with higher genetic diversity ( p & lt ; 0.001 ) , complexity ( p = 0.009 ) , and Shannon entropy ( p = 0.022 ) , but not with length variation ( p = 0.111 ) .
	manualset3
215469	3	419830	7	NULL	NULL	NULL	NULL	HIV diversity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	HRM scores were also compared to sequenced-based measures of HIV diversity ; higher HRM scores were associated with higher genetic diversity ( p & lt ; 0.001 ) , complexity ( p = 0.009 ) , and Shannon entropy ( p = 0.022 ) , but not with length variation ( p = 0.111 ) .
	manualset3
215470	4	419830	7	NULL	NULL	0	NULL	 higher HRM scores	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	HRM scores were also compared to sequenced-based measures of HIV diversity ; higher HRM scores were associated with higher genetic diversity ( p & lt ; 0.001 ) , complexity ( p = 0.009 ) , and Shannon entropy ( p = 0.022 ) , but not with length variation ( p = 0.111 ) .
	manualset3
215471	5	419830	7	NULL	NULL	0	NULL	higher genetic diversity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	HRM scores were also compared to sequenced-based measures of HIV diversity ; higher HRM scores were associated with higher genetic diversity ( p & lt ; 0.001 ) , complexity ( p = 0.009 ) , and Shannon entropy ( p = 0.022 ) , but not with length variation ( p = 0.111 ) .
	manualset3
215472	6	419830	7	NULL	NULL	0	NULL	p & lt ; 0.001	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	HRM scores were also compared to sequenced-based measures of HIV diversity ; higher HRM scores were associated with higher genetic diversity ( p & lt ; 0.001 ) , complexity ( p = 0.009 ) , and Shannon entropy ( p = 0.022 ) , but not with length variation ( p = 0.111 ) .
	manualset3
215473	7	419830	7	NULL	NULL	0	NULL	complexity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	HRM scores were also compared to sequenced-based measures of HIV diversity ; higher HRM scores were associated with higher genetic diversity ( p & lt ; 0.001 ) , complexity ( p = 0.009 ) , and Shannon entropy ( p = 0.022 ) , but not with length variation ( p = 0.111 ) .
	manualset3
215474	8	419830	7	NULL	NULL	0	NULL	 p = 0.009	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	HRM scores were also compared to sequenced-based measures of HIV diversity ; higher HRM scores were associated with higher genetic diversity ( p & lt ; 0.001 ) , complexity ( p = 0.009 ) , and Shannon entropy ( p = 0.022 ) , but not with length variation ( p = 0.111 ) .
	manualset3
215475	9	419830	7	NULL	NULL	0	NULL	Shannon entropy	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	HRM scores were also compared to sequenced-based measures of HIV diversity ; higher HRM scores were associated with higher genetic diversity ( p & lt ; 0.001 ) , complexity ( p = 0.009 ) , and Shannon entropy ( p = 0.022 ) , but not with length variation ( p = 0.111 ) .
	manualset3
215476	10	419830	7	NULL	NULL	0	NULL	 p = 0.022	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	HRM scores were also compared to sequenced-based measures of HIV diversity ; higher HRM scores were associated with higher genetic diversity ( p & lt ; 0.001 ) , complexity ( p = 0.009 ) , and Shannon entropy ( p = 0.022 ) , but not with length variation ( p = 0.111 ) .
	manualset3
215477	11	419830	7	NULL	NULL	0	NULL	length variation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	HRM scores were also compared to sequenced-based measures of HIV diversity ; higher HRM scores were associated with higher genetic diversity ( p & lt ; 0.001 ) , complexity ( p = 0.009 ) , and Shannon entropy ( p = 0.022 ) , but not with length variation ( p = 0.111 ) .
	manualset3
215478	12	419830	7	NULL	NULL	0	NULL	p = 0.111	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	HRM scores were also compared to sequenced-based measures of HIV diversity ; higher HRM scores were associated with higher genetic diversity ( p & lt ; 0.001 ) , complexity ( p = 0.009 ) , and Shannon entropy ( p = 0.022 ) , but not with length variation ( p = 0.111 ) .
	manualset3
215488	1	419831	7	NULL	NULL	0	NULL	6S RNA sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the 6S RNA sequences from P. aeruginosa and E. coli share only a 60.4 % homology , we are able to propose a common secondary structural model .
	manualset3
215489	2	419831	7	NULL	NULL	0	NULL	P. aeruginosa	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the 6S RNA sequences from P. aeruginosa and E. coli share only a 60.4 % homology , we are able to propose a common secondary structural model .
	manualset3
215490	3	419831	7	NULL	NULL	0	NULL	E. coli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the 6S RNA sequences from P. aeruginosa and E. coli share only a 60.4 % homology , we are able to propose a common secondary structural model .
	manualset3
215491	4	419831	7	NULL	NULL	0	NULL	60.4 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the 6S RNA sequences from P. aeruginosa and E. coli share only a 60.4 % homology , we are able to propose a common secondary structural model .
	manualset3
215492	5	419831	7	NULL	NULL	0	NULL	homology	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the 6S RNA sequences from P. aeruginosa and E. coli share only a 60.4 % homology , we are able to propose a common secondary structural model .
	manualset3
215493	6	419831	7	NULL	NULL	0	NULL	common secondary structural model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the 6S RNA sequences from P. aeruginosa and E. coli share only a 60.4 % homology , we are able to propose a common secondary structural model .
	manualset3
215494	1	419832	7	NULL	NULL	0	NULL	striatum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Throughout most of the striatum , cerebral cortex and limbic system , the diffuse , even neuropil staining produced by the Timm-Danscher method was mirrored by comparable fluorescence in TSQ-stained sections .
	manualset3
215495	2	419832	7	NULL	NULL	0	NULL	cerebral cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Throughout most of the striatum , cerebral cortex and limbic system , the diffuse , even neuropil staining produced by the Timm-Danscher method was mirrored by comparable fluorescence in TSQ-stained sections .
	manualset3
215496	3	419832	7	NULL	NULL	0	NULL	limbic system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Throughout most of the striatum , cerebral cortex and limbic system , the diffuse , even neuropil staining produced by the Timm-Danscher method was mirrored by comparable fluorescence in TSQ-stained sections .
	manualset3
215497	4	419832	7	NULL	NULL	0	NULL	neuropil staining 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Throughout most of the striatum , cerebral cortex and limbic system , the diffuse , even neuropil staining produced by the Timm-Danscher method was mirrored by comparable fluorescence in TSQ-stained sections .
	manualset3
215498	5	419832	7	NULL	NULL	0	NULL	 Timm-Danscher method 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Throughout most of the striatum , cerebral cortex and limbic system , the diffuse , even neuropil staining produced by the Timm-Danscher method was mirrored by comparable fluorescence in TSQ-stained sections .
	manualset3
215499	6	419832	7	NULL	NULL	0	NULL	comparable fluorescence	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Throughout most of the striatum , cerebral cortex and limbic system , the diffuse , even neuropil staining produced by the Timm-Danscher method was mirrored by comparable fluorescence in TSQ-stained sections .
	manualset3
215500	7	419832	7	NULL	NULL	0	NULL	TSQ-stained sections	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Throughout most of the striatum , cerebral cortex and limbic system , the diffuse , even neuropil staining produced by the Timm-Danscher method was mirrored by comparable fluorescence in TSQ-stained sections .
	manualset3
215501	1	419833	7	NULL	NULL	0	NULL	Clinician 's guide	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinician 's guide to nuclear medicine imaging procedures .
	manualset3
215502	2	419833	7	NULL	NULL	0	NULL	nuclear medicine imaging procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinician 's guide to nuclear medicine imaging procedures .
	manualset3
215503	1	419834	7	NULL	NULL	0	NULL	methods	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	All these methods are applied to the foetal-ECG extraction problem by using real ECG data .
	manualset3
215504	2	419834	7	NULL	NULL	0	NULL	foetal-ECG extraction problem	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All these methods are applied to the foetal-ECG extraction problem by using real ECG data .
	manualset3
215505	3	419834	7	NULL	NULL	NULL	NULL	real ECG data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	All these methods are applied to the foetal-ECG extraction problem by using real ECG data .
	manualset3
215506	1	419835	7	NULL	NULL	0	NULL	compost 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	With compost , 23 % of the labeled anthracene was transformed into 14CO2 and 42 % was fixed to the soil matrix irreversibly .
	manualset3
215507	2	419835	7	NULL	NULL	0	NULL	23 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With compost , 23 % of the labeled anthracene was transformed into 14CO2 and 42 % was fixed to the soil matrix irreversibly .
	manualset3
215508	3	419835	7	NULL	NULL	0	NULL	labeled anthracene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	With compost , 23 % of the labeled anthracene was transformed into 14CO2 and 42 % was fixed to the soil matrix irreversibly .
	manualset3
215509	4	419835	7	NULL	NULL	0	NULL	14CO2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	With compost , 23 % of the labeled anthracene was transformed into 14CO2 and 42 % was fixed to the soil matrix irreversibly .
	manualset3
215510	5	419835	7	NULL	NULL	0	NULL	42 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With compost , 23 % of the labeled anthracene was transformed into 14CO2 and 42 % was fixed to the soil matrix irreversibly .
	manualset3
215511	6	419835	7	NULL	NULL	0	NULL	soil matrix 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	With compost , 23 % of the labeled anthracene was transformed into 14CO2 and 42 % was fixed to the soil matrix irreversibly .
	manualset3
215512	1	419836	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This study 1 ) assessed total mercury levels in both random urine specimens from pregnant women , and in cord blood ; and 2 ) examined environmental sources of exposure from a convenience sample in a predominantly Caribbean immigrant population in Brooklyn , New York .
	manualset3
215513	2	419836	7	NULL	NULL	0	NULL	total mercury levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This study 1 ) assessed total mercury levels in both random urine specimens from pregnant women , and in cord blood ; and 2 ) examined environmental sources of exposure from a convenience sample in a predominantly Caribbean immigrant population in Brooklyn , New York .
	manualset3
215514	3	419836	7	NULL	NULL	0	NULL	random urine specimens	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	This study 1 ) assessed total mercury levels in both random urine specimens from pregnant women , and in cord blood ; and 2 ) examined environmental sources of exposure from a convenience sample in a predominantly Caribbean immigrant population in Brooklyn , New York .
	manualset3
215515	4	419836	7	NULL	NULL	0	NULL	pregnant women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This study 1 ) assessed total mercury levels in both random urine specimens from pregnant women , and in cord blood ; and 2 ) examined environmental sources of exposure from a convenience sample in a predominantly Caribbean immigrant population in Brooklyn , New York .
	manualset3
215516	5	419836	7	NULL	NULL	0	NULL	cord blood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This study 1 ) assessed total mercury levels in both random urine specimens from pregnant women , and in cord blood ; and 2 ) examined environmental sources of exposure from a convenience sample in a predominantly Caribbean immigrant population in Brooklyn , New York .
	manualset3
215517	6	419836	7	NULL	NULL	0	NULL	environmental sources	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	This study 1 ) assessed total mercury levels in both random urine specimens from pregnant women , and in cord blood ; and 2 ) examined environmental sources of exposure from a convenience sample in a predominantly Caribbean immigrant population in Brooklyn , New York .
	manualset3
215518	7	419836	7	NULL	NULL	0	NULL	convenience sample	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	This study 1 ) assessed total mercury levels in both random urine specimens from pregnant women , and in cord blood ; and 2 ) examined environmental sources of exposure from a convenience sample in a predominantly Caribbean immigrant population in Brooklyn , New York .
	manualset3
215519	8	419836	7	NULL	NULL	0	NULL	Caribbean immigrant population 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This study 1 ) assessed total mercury levels in both random urine specimens from pregnant women , and in cord blood ; and 2 ) examined environmental sources of exposure from a convenience sample in a predominantly Caribbean immigrant population in Brooklyn , New York .
	manualset3
215520	9	419836	7	NULL	NULL	0	NULL	Brooklyn , New York 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	This study 1 ) assessed total mercury levels in both random urine specimens from pregnant women , and in cord blood ; and 2 ) examined environmental sources of exposure from a convenience sample in a predominantly Caribbean immigrant population in Brooklyn , New York .
	manualset3
216724	10	419836	7	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This study 1 ) assessed total mercury levels in both random urine specimens from pregnant women , and in cord blood ; and 2 ) examined environmental sources of exposure from a convenience sample in a predominantly Caribbean immigrant population in Brooklyn , New York .
	manualset3
215521	1	419837	7	NULL	NULL	0	NULL	Assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Assays may be performed either on selected islets or on aliquots of semi-purified preparations designated for grafting , allowing thus the rapid estimation of graft function of the entire preparation .
	manualset3
215522	2	419837	7	NULL	NULL	NULL	NULL	selected islets	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Assays may be performed either on selected islets or on aliquots of semi-purified preparations designated for grafting , allowing thus the rapid estimation of graft function of the entire preparation .
	manualset3
215523	3	419837	7	NULL	NULL	0	NULL	 aliquots	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Assays may be performed either on selected islets or on aliquots of semi-purified preparations designated for grafting , allowing thus the rapid estimation of graft function of the entire preparation .
	manualset3
215524	4	419837	7	NULL	NULL	0	NULL	semi-purified preparations	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Assays may be performed either on selected islets or on aliquots of semi-purified preparations designated for grafting , allowing thus the rapid estimation of graft function of the entire preparation .
	manualset3
215525	5	419837	7	NULL	NULL	0	NULL	grafting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Assays may be performed either on selected islets or on aliquots of semi-purified preparations designated for grafting , allowing thus the rapid estimation of graft function of the entire preparation .
	manualset3
215526	6	419837	7	NULL	NULL	0	NULL	 rapid estimation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Assays may be performed either on selected islets or on aliquots of semi-purified preparations designated for grafting , allowing thus the rapid estimation of graft function of the entire preparation .
	manualset3
215527	7	419837	7	NULL	NULL	0	NULL	graft function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Assays may be performed either on selected islets or on aliquots of semi-purified preparations designated for grafting , allowing thus the rapid estimation of graft function of the entire preparation .
	manualset3
215528	8	419837	7	NULL	NULL	0	NULL	entire preparation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Assays may be performed either on selected islets or on aliquots of semi-purified preparations designated for grafting , allowing thus the rapid estimation of graft function of the entire preparation .
	manualset3
215529	1	419838	7	NULL	NULL	0	NULL	 Cr layer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the Cr layer is insensitive to hydrogen , it enables the formation of a network of continuous Pd/Cr nanowires with thicknesses of the Pd layer as thin as 2 nm .
	manualset3
215530	2	419838	7	NULL	NULL	0	NULL	hydrogen	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the Cr layer is insensitive to hydrogen , it enables the formation of a network of continuous Pd/Cr nanowires with thicknesses of the Pd layer as thin as 2 nm .
	manualset3
215531	3	419838	7	NULL	NULL	0	NULL	formation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the Cr layer is insensitive to hydrogen , it enables the formation of a network of continuous Pd/Cr nanowires with thicknesses of the Pd layer as thin as 2 nm .
	manualset3
215532	4	419838	7	NULL	NULL	NULL	NULL	continuous Pd/Cr nanowires	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although the Cr layer is insensitive to hydrogen , it enables the formation of a network of continuous Pd/Cr nanowires with thicknesses of the Pd layer as thin as 2 nm .
	manualset3
215533	5	419838	7	NULL	NULL	0	NULL	thicknesses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the Cr layer is insensitive to hydrogen , it enables the formation of a network of continuous Pd/Cr nanowires with thicknesses of the Pd layer as thin as 2 nm .
	manualset3
215534	6	419838	7	NULL	NULL	0	NULL	Pd layer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the Cr layer is insensitive to hydrogen , it enables the formation of a network of continuous Pd/Cr nanowires with thicknesses of the Pd layer as thin as 2 nm .
	manualset3
215535	7	419838	7	NULL	NULL	0	NULL	2 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the Cr layer is insensitive to hydrogen , it enables the formation of a network of continuous Pd/Cr nanowires with thicknesses of the Pd layer as thin as 2 nm .
	manualset3
216725	8	419838	7	NULL	NULL	NULL	NULL	network	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although the Cr layer is insensitive to hydrogen , it enables the formation of a network of continuous Pd/Cr nanowires with thicknesses of the Pd layer as thin as 2 nm .
	manualset3
215536	1	419839	7	NULL	NULL	0	NULL	Mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations of the BRAF gene were found in the SNU-80 ( G468R ) and the SNU-790 ( V599E ) cell lines , but no mutations in the K-ras gene were present .
	manualset3
215537	2	419839	7	NULL	NULL	0	NULL	BRAF gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations of the BRAF gene were found in the SNU-80 ( G468R ) and the SNU-790 ( V599E ) cell lines , but no mutations in the K-ras gene were present .
	manualset3
215538	3	419839	7	NULL	NULL	0	NULL	SNU-80 ( G468R ) cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations of the BRAF gene were found in the SNU-80 ( G468R ) and the SNU-790 ( V599E ) cell lines , but no mutations in the K-ras gene were present .
	manualset3
215539	4	419839	7	NULL	NULL	0	NULL	SNU-790 ( V599E ) cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations of the BRAF gene were found in the SNU-80 ( G468R ) and the SNU-790 ( V599E ) cell lines , but no mutations in the K-ras gene were present .
	manualset3
215540	5	419839	7	NULL	NULL	0	NULL	no mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations of the BRAF gene were found in the SNU-80 ( G468R ) and the SNU-790 ( V599E ) cell lines , but no mutations in the K-ras gene were present .
	manualset3
215541	6	419839	7	NULL	NULL	0	NULL	K-ras gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations of the BRAF gene were found in the SNU-80 ( G468R ) and the SNU-790 ( V599E ) cell lines , but no mutations in the K-ras gene were present .
	manualset3
215542	1	419840	7	NULL	NULL	0	NULL	China 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In China , the care of patients with a bleeding disorder is not organized into designated centers with a national protocol .
	manualset3
215543	2	419840	7	NULL	NULL	0	NULL	care	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In China , the care of patients with a bleeding disorder is not organized into designated centers with a national protocol .
	manualset3
215544	3	419840	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In China , the care of patients with a bleeding disorder is not organized into designated centers with a national protocol .
	manualset3
215545	4	419840	7	NULL	NULL	0	NULL	bleeding disorder	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In China , the care of patients with a bleeding disorder is not organized into designated centers with a national protocol .
	manualset3
215546	5	419840	7	NULL	NULL	0	NULL	designated centers	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In China , the care of patients with a bleeding disorder is not organized into designated centers with a national protocol .
	manualset3
215547	6	419840	7	NULL	NULL	0	NULL	national protocol	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In China , the care of patients with a bleeding disorder is not organized into designated centers with a national protocol .
	manualset3
215548	1	419841	7	NULL	NULL	0	NULL	D. melanogaster	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We find that , as in D. melanogaster , there is an excess of genes duplicated from the X chromosome across the genus Drosophila .
	manualset3
215549	2	419841	7	NULL	NULL	0	NULL	excess of genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We find that , as in D. melanogaster , there is an excess of genes duplicated from the X chromosome across the genus Drosophila .
	manualset3
215550	3	419841	7	NULL	NULL	0	NULL	X chromosome	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	We find that , as in D. melanogaster , there is an excess of genes duplicated from the X chromosome across the genus Drosophila .
	manualset3
215551	4	419841	7	NULL	NULL	0	NULL	genus Drosophila	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We find that , as in D. melanogaster , there is an excess of genes duplicated from the X chromosome across the genus Drosophila .
	manualset3
215552	1	419842	7	NULL	NULL	0	NULL	reaction rate constants	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction rate constants of N3 x with malatonin and chloromelatonin are 9.8 x 10 ( 9 ) M-1 s-1 and 3.5 x 10 ( 9 ) M-1 s-1 and 3.5 x 10 ( 9 ) M-1 s-1 , respectively .
	manualset3
215553	2	419842	7	NULL	NULL	0	NULL	N3 x	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction rate constants of N3 x with malatonin and chloromelatonin are 9.8 x 10 ( 9 ) M-1 s-1 and 3.5 x 10 ( 9 ) M-1 s-1 and 3.5 x 10 ( 9 ) M-1 s-1 , respectively .
	manualset3
215554	3	419842	7	NULL	NULL	0	NULL	malatonin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction rate constants of N3 x with malatonin and chloromelatonin are 9.8 x 10 ( 9 ) M-1 s-1 and 3.5 x 10 ( 9 ) M-1 s-1 and 3.5 x 10 ( 9 ) M-1 s-1 , respectively .
	manualset3
215555	4	419842	7	NULL	NULL	0	NULL	chloromelatonin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction rate constants of N3 x with malatonin and chloromelatonin are 9.8 x 10 ( 9 ) M-1 s-1 and 3.5 x 10 ( 9 ) M-1 s-1 and 3.5 x 10 ( 9 ) M-1 s-1 , respectively .
	manualset3
215556	5	419842	7	NULL	NULL	0	NULL	9.8 x 10 ( 9 ) M-1 s-1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction rate constants of N3 x with malatonin and chloromelatonin are 9.8 x 10 ( 9 ) M-1 s-1 and 3.5 x 10 ( 9 ) M-1 s-1 and 3.5 x 10 ( 9 ) M-1 s-1 , respectively .
	manualset3
215557	6	419842	7	NULL	NULL	0	NULL	3.5 x 10 ( 9 ) M-1 s-1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction rate constants of N3 x with malatonin and chloromelatonin are 9.8 x 10 ( 9 ) M-1 s-1 and 3.5 x 10 ( 9 ) M-1 s-1 and 3.5 x 10 ( 9 ) M-1 s-1 , respectively .
	manualset3
215558	7	419842	7	NULL	NULL	0	NULL	3.5 x 10 ( 9 ) M-1 s-1 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The reaction rate constants of N3 x with malatonin and chloromelatonin are 9.8 x 10 ( 9 ) M-1 s-1 and 3.5 x 10 ( 9 ) M-1 s-1 and 3.5 x 10 ( 9 ) M-1 s-1 , respectively .
	manualset3
215559	1	419843	7	NULL	NULL	NULL	NULL	lanthanide chelating tag ( M8 )	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A new lanthanide chelating tag ( M8 ) for paramagnetic labeling of biomolecules is presented , which is based on an eight-fold , stereoselectively methyl-substituted DOTA that can be covalently linked to the host molecule by a single disulfide bond .
	manualset3
215560	2	419843	7	NULL	NULL	0	NULL	paramagnetic labeling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A new lanthanide chelating tag ( M8 ) for paramagnetic labeling of biomolecules is presented , which is based on an eight-fold , stereoselectively methyl-substituted DOTA that can be covalently linked to the host molecule by a single disulfide bond .
	manualset3
215561	3	419843	7	NULL	NULL	0	NULL	biomolecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A new lanthanide chelating tag ( M8 ) for paramagnetic labeling of biomolecules is presented , which is based on an eight-fold , stereoselectively methyl-substituted DOTA that can be covalently linked to the host molecule by a single disulfide bond .
	manualset3
215562	4	419843	7	NULL	NULL	0	NULL	eight-fold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new lanthanide chelating tag ( M8 ) for paramagnetic labeling of biomolecules is presented , which is based on an eight-fold , stereoselectively methyl-substituted DOTA that can be covalently linked to the host molecule by a single disulfide bond .
	manualset3
215563	5	419843	7	NULL	NULL	0	NULL	stereoselectively methyl-substituted DOTA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A new lanthanide chelating tag ( M8 ) for paramagnetic labeling of biomolecules is presented , which is based on an eight-fold , stereoselectively methyl-substituted DOTA that can be covalently linked to the host molecule by a single disulfide bond .
	manualset3
215564	6	419843	7	NULL	NULL	0	NULL	host molecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	A new lanthanide chelating tag ( M8 ) for paramagnetic labeling of biomolecules is presented , which is based on an eight-fold , stereoselectively methyl-substituted DOTA that can be covalently linked to the host molecule by a single disulfide bond .
	manualset3
215565	7	419843	7	NULL	NULL	0	NULL	 single disulfide bond	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A new lanthanide chelating tag ( M8 ) for paramagnetic labeling of biomolecules is presented , which is based on an eight-fold , stereoselectively methyl-substituted DOTA that can be covalently linked to the host molecule by a single disulfide bond .
	manualset3
215566	1	419844	7	NULL	NULL	0	NULL	categorical nature	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The categorical nature of cow-SCC can be utilized by deriving new traits such as the fraction of cow-SCC records in a lactation that are associated with an infection with a major pathogen .
	manualset3
215567	2	419844	7	NULL	NULL	0	NULL	cow-SCC	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The categorical nature of cow-SCC can be utilized by deriving new traits such as the fraction of cow-SCC records in a lactation that are associated with an infection with a major pathogen .
	manualset3
215568	3	419844	7	NULL	NULL	NULL	NULL	 new traits	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The categorical nature of cow-SCC can be utilized by deriving new traits such as the fraction of cow-SCC records in a lactation that are associated with an infection with a major pathogen .
	manualset3
215569	4	419844	7	NULL	NULL	0	NULL	fraction 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The categorical nature of cow-SCC can be utilized by deriving new traits such as the fraction of cow-SCC records in a lactation that are associated with an infection with a major pathogen .
	manualset3
215570	5	419844	7	NULL	NULL	0	NULL	cow-SCC records	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The categorical nature of cow-SCC can be utilized by deriving new traits such as the fraction of cow-SCC records in a lactation that are associated with an infection with a major pathogen .
	manualset3
215571	6	419844	7	NULL	NULL	0	NULL	lactation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The categorical nature of cow-SCC can be utilized by deriving new traits such as the fraction of cow-SCC records in a lactation that are associated with an infection with a major pathogen .
	manualset3
215572	7	419844	7	NULL	NULL	0	NULL	 infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The categorical nature of cow-SCC can be utilized by deriving new traits such as the fraction of cow-SCC records in a lactation that are associated with an infection with a major pathogen .
	manualset3
215573	8	419844	7	NULL	NULL	0	NULL	major pathogen	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The categorical nature of cow-SCC can be utilized by deriving new traits such as the fraction of cow-SCC records in a lactation that are associated with an infection with a major pathogen .
	manualset3
215574	1	419845	7	NULL	NULL	0	NULL	 conclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , in our study group MRI detected PVT in all liver transplant recipients requiring jump grafts at transplantation .
	manualset3
215575	2	419845	7	NULL	NULL	0	NULL	study group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , in our study group MRI detected PVT in all liver transplant recipients requiring jump grafts at transplantation .
	manualset3
215576	3	419845	7	NULL	NULL	0	NULL	MRI	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , in our study group MRI detected PVT in all liver transplant recipients requiring jump grafts at transplantation .
	manualset3
215577	4	419845	7	NULL	NULL	0	NULL	PVT	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , in our study group MRI detected PVT in all liver transplant recipients requiring jump grafts at transplantation .
	manualset3
215578	5	419845	7	NULL	NULL	0	NULL	liver transplant recipients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , in our study group MRI detected PVT in all liver transplant recipients requiring jump grafts at transplantation .
	manualset3
215579	6	419845	7	NULL	NULL	0	NULL	jump grafts 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , in our study group MRI detected PVT in all liver transplant recipients requiring jump grafts at transplantation .
	manualset3
215580	7	419845	7	NULL	NULL	0	NULL	transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , in our study group MRI detected PVT in all liver transplant recipients requiring jump grafts at transplantation .
	manualset3
215581	1	419846	7	NULL	NULL	0	NULL	construction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , the construction of chimeras between quail and chick has been a turning point , instrumental in appraising the contribution of the cephalic neural crest to the development of ocular and periocular structures .
	manualset3
215582	2	419846	7	NULL	NULL	0	NULL	chimeras	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , the construction of chimeras between quail and chick has been a turning point , instrumental in appraising the contribution of the cephalic neural crest to the development of ocular and periocular structures .
	manualset3
215583	3	419846	7	NULL	NULL	0	NULL	quail 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , the construction of chimeras between quail and chick has been a turning point , instrumental in appraising the contribution of the cephalic neural crest to the development of ocular and periocular structures .
	manualset3
215584	4	419846	7	NULL	NULL	0	NULL	chick	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , the construction of chimeras between quail and chick has been a turning point , instrumental in appraising the contribution of the cephalic neural crest to the development of ocular and periocular structures .
	manualset3
215585	5	419846	7	NULL	NULL	0	NULL	turning point	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , the construction of chimeras between quail and chick has been a turning point , instrumental in appraising the contribution of the cephalic neural crest to the development of ocular and periocular structures .
	manualset3
215586	6	419846	7	NULL	NULL	0	NULL	contribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , the construction of chimeras between quail and chick has been a turning point , instrumental in appraising the contribution of the cephalic neural crest to the development of ocular and periocular structures .
	manualset3
215587	7	419846	7	NULL	NULL	0	NULL	cephalic neural crest	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , the construction of chimeras between quail and chick has been a turning point , instrumental in appraising the contribution of the cephalic neural crest to the development of ocular and periocular structures .
	manualset3
215588	8	419846	7	NULL	NULL	0	NULL	 development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this respect , the construction of chimeras between quail and chick has been a turning point , instrumental in appraising the contribution of the cephalic neural crest to the development of ocular and periocular structures .
	manualset3
215589	9	419846	7	NULL	NULL	NULL	NULL	ocular structures	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this respect , the construction of chimeras between quail and chick has been a turning point , instrumental in appraising the contribution of the cephalic neural crest to the development of ocular and periocular structures .
	manualset3
215590	10	419846	7	NULL	NULL	NULL	NULL	periocular structures	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this respect , the construction of chimeras between quail and chick has been a turning point , instrumental in appraising the contribution of the cephalic neural crest to the development of ocular and periocular structures .
	manualset3
215591	1	419847	7	NULL	NULL	0	NULL	excretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The excretion of radioactivity in the bile within 48 h after the oral administration of 14C-NS-49 ( 1 mg/kg ) was 5.9 % of the dose , and the excretion of radioactivity in the exhaled air after the intravenous administration ( 0.2 mg/kg ) was negligible .
	manualset3
215592	2	419847	7	NULL	NULL	0	NULL	radioactivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The excretion of radioactivity in the bile within 48 h after the oral administration of 14C-NS-49 ( 1 mg/kg ) was 5.9 % of the dose , and the excretion of radioactivity in the exhaled air after the intravenous administration ( 0.2 mg/kg ) was negligible .
	manualset3
215593	3	419847	7	NULL	NULL	0	NULL	 bile	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The excretion of radioactivity in the bile within 48 h after the oral administration of 14C-NS-49 ( 1 mg/kg ) was 5.9 % of the dose , and the excretion of radioactivity in the exhaled air after the intravenous administration ( 0.2 mg/kg ) was negligible .
	manualset3
215594	4	419847	7	NULL	NULL	0	NULL	48 h 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The excretion of radioactivity in the bile within 48 h after the oral administration of 14C-NS-49 ( 1 mg/kg ) was 5.9 % of the dose , and the excretion of radioactivity in the exhaled air after the intravenous administration ( 0.2 mg/kg ) was negligible .
	manualset3
215595	5	419847	7	NULL	NULL	0	NULL	oral administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The excretion of radioactivity in the bile within 48 h after the oral administration of 14C-NS-49 ( 1 mg/kg ) was 5.9 % of the dose , and the excretion of radioactivity in the exhaled air after the intravenous administration ( 0.2 mg/kg ) was negligible .
	manualset3
215596	6	419847	7	NULL	NULL	0	NULL	14C-NS-49 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The excretion of radioactivity in the bile within 48 h after the oral administration of 14C-NS-49 ( 1 mg/kg ) was 5.9 % of the dose , and the excretion of radioactivity in the exhaled air after the intravenous administration ( 0.2 mg/kg ) was negligible .
	manualset3
215597	7	419847	7	NULL	NULL	0	NULL	1 mg/kg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The excretion of radioactivity in the bile within 48 h after the oral administration of 14C-NS-49 ( 1 mg/kg ) was 5.9 % of the dose , and the excretion of radioactivity in the exhaled air after the intravenous administration ( 0.2 mg/kg ) was negligible .
	manualset3
215598	8	419847	7	NULL	NULL	0	NULL	 5.9 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The excretion of radioactivity in the bile within 48 h after the oral administration of 14C-NS-49 ( 1 mg/kg ) was 5.9 % of the dose , and the excretion of radioactivity in the exhaled air after the intravenous administration ( 0.2 mg/kg ) was negligible .
	manualset3
215599	9	419847	7	NULL	NULL	0	NULL	dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The excretion of radioactivity in the bile within 48 h after the oral administration of 14C-NS-49 ( 1 mg/kg ) was 5.9 % of the dose , and the excretion of radioactivity in the exhaled air after the intravenous administration ( 0.2 mg/kg ) was negligible .
	manualset3
215600	10	419847	7	NULL	NULL	0	NULL	excretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The excretion of radioactivity in the bile within 48 h after the oral administration of 14C-NS-49 ( 1 mg/kg ) was 5.9 % of the dose , and the excretion of radioactivity in the exhaled air after the intravenous administration ( 0.2 mg/kg ) was negligible .
	manualset3
215601	11	419847	7	NULL	NULL	0	NULL	radioactivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The excretion of radioactivity in the bile within 48 h after the oral administration of 14C-NS-49 ( 1 mg/kg ) was 5.9 % of the dose , and the excretion of radioactivity in the exhaled air after the intravenous administration ( 0.2 mg/kg ) was negligible .
	manualset3
215602	12	419847	7	NULL	NULL	0	NULL	exhaled air	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The excretion of radioactivity in the bile within 48 h after the oral administration of 14C-NS-49 ( 1 mg/kg ) was 5.9 % of the dose , and the excretion of radioactivity in the exhaled air after the intravenous administration ( 0.2 mg/kg ) was negligible .
	manualset3
215603	13	419847	7	NULL	NULL	0	NULL	intravenous administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The excretion of radioactivity in the bile within 48 h after the oral administration of 14C-NS-49 ( 1 mg/kg ) was 5.9 % of the dose , and the excretion of radioactivity in the exhaled air after the intravenous administration ( 0.2 mg/kg ) was negligible .
	manualset3
215604	14	419847	7	NULL	NULL	0	NULL	 0.2 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The excretion of radioactivity in the bile within 48 h after the oral administration of 14C-NS-49 ( 1 mg/kg ) was 5.9 % of the dose , and the excretion of radioactivity in the exhaled air after the intravenous administration ( 0.2 mg/kg ) was negligible .
	manualset3
215605	1	419848	7	NULL	NULL	0	NULL	TCR - chain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the TCR - chain is invariant , NKT TCR V exhibits greater diversity , with one ( V11 ) and three ( V8 , V7 , and V2 ) V chains in humans and mice , respectively .
	manualset3
215606	2	419848	7	NULL	NULL	0	NULL	NKT TCR V	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the TCR - chain is invariant , NKT TCR V exhibits greater diversity , with one ( V11 ) and three ( V8 , V7 , and V2 ) V chains in humans and mice , respectively .
	manualset3
215607	3	419848	7	NULL	NULL	0	NULL	one 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the TCR - chain is invariant , NKT TCR V exhibits greater diversity , with one ( V11 ) and three ( V8 , V7 , and V2 ) V chains in humans and mice , respectively .
	manualset3
215608	4	419848	7	NULL	NULL	0	NULL	( V11 ) V chains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the TCR - chain is invariant , NKT TCR V exhibits greater diversity , with one ( V11 ) and three ( V8 , V7 , and V2 ) V chains in humans and mice , respectively .
	manualset3
215609	5	419848	7	NULL	NULL	0	NULL	 three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the TCR - chain is invariant , NKT TCR V exhibits greater diversity , with one ( V11 ) and three ( V8 , V7 , and V2 ) V chains in humans and mice , respectively .
	manualset3
215610	6	419848	7	NULL	NULL	0	NULL	V8 V chains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the TCR - chain is invariant , NKT TCR V exhibits greater diversity , with one ( V11 ) and three ( V8 , V7 , and V2 ) V chains in humans and mice , respectively .
	manualset3
215611	7	419848	7	NULL	NULL	0	NULL	V7 V chains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the TCR - chain is invariant , NKT TCR V exhibits greater diversity , with one ( V11 ) and three ( V8 , V7 , and V2 ) V chains in humans and mice , respectively .
	manualset3
215612	8	419848	7	NULL	NULL	0	NULL	V2  V chains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the TCR - chain is invariant , NKT TCR V exhibits greater diversity , with one ( V11 ) and three ( V8 , V7 , and V2 ) V chains in humans and mice , respectively .
	manualset3
215613	9	419848	7	NULL	NULL	0	NULL	humans 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the TCR - chain is invariant , NKT TCR V exhibits greater diversity , with one ( V11 ) and three ( V8 , V7 , and V2 ) V chains in humans and mice , respectively .
	manualset3
215614	10	419848	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the TCR - chain is invariant , NKT TCR V exhibits greater diversity , with one ( V11 ) and three ( V8 , V7 , and V2 ) V chains in humans and mice , respectively .
	manualset3
215615	1	419849	7	NULL	NULL	0	NULL	functional core	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The functional core of these molecules is stabilized by a diverse set of tertiary interaction motifs that often bring together distant regions of conserved nucleotides .
	manualset3
215616	2	419849	7	NULL	NULL	0	NULL	molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The functional core of these molecules is stabilized by a diverse set of tertiary interaction motifs that often bring together distant regions of conserved nucleotides .
	manualset3
215617	3	419849	7	NULL	NULL	0	NULL	diverse set	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The functional core of these molecules is stabilized by a diverse set of tertiary interaction motifs that often bring together distant regions of conserved nucleotides .
	manualset3
215618	4	419849	7	NULL	NULL	0	NULL	tertiary interaction motifs	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The functional core of these molecules is stabilized by a diverse set of tertiary interaction motifs that often bring together distant regions of conserved nucleotides .
	manualset3
215619	5	419849	7	NULL	NULL	0	NULL	distant regions	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The functional core of these molecules is stabilized by a diverse set of tertiary interaction motifs that often bring together distant regions of conserved nucleotides .
	manualset3
215620	6	419849	7	NULL	NULL	0	NULL	conserved nucleotides	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The functional core of these molecules is stabilized by a diverse set of tertiary interaction motifs that often bring together distant regions of conserved nucleotides .
	manualset3
215621	1	419850	7	NULL	NULL	0	NULL	BHK cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In BHK cells labeled to equilibrium with ( 3H ) choline and treated with sphingomyelinase the surface pool of sphingomyelin is degraded very rapidly ( half-time 10 min ) but the internal pool of sphingomyelin which accounts for about 30 % of the total is only degraded slowly ( half-time about 80 h ) showing that the internal pool does not normally reach the surface .
	manualset3
215622	2	419850	7	NULL	NULL	0	NULL	( 3H ) choline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In BHK cells labeled to equilibrium with ( 3H ) choline and treated with sphingomyelinase the surface pool of sphingomyelin is degraded very rapidly ( half-time 10 min ) but the internal pool of sphingomyelin which accounts for about 30 % of the total is only degraded slowly ( half-time about 80 h ) showing that the internal pool does not normally reach the surface .
	manualset3
215623	3	419850	7	NULL	NULL	0	NULL	sphingomyelinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In BHK cells labeled to equilibrium with ( 3H ) choline and treated with sphingomyelinase the surface pool of sphingomyelin is degraded very rapidly ( half-time 10 min ) but the internal pool of sphingomyelin which accounts for about 30 % of the total is only degraded slowly ( half-time about 80 h ) showing that the internal pool does not normally reach the surface .
	manualset3
215624	4	419850	7	NULL	NULL	0	NULL	surface pool	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In BHK cells labeled to equilibrium with ( 3H ) choline and treated with sphingomyelinase the surface pool of sphingomyelin is degraded very rapidly ( half-time 10 min ) but the internal pool of sphingomyelin which accounts for about 30 % of the total is only degraded slowly ( half-time about 80 h ) showing that the internal pool does not normally reach the surface .
	manualset3
215625	5	419850	7	NULL	NULL	0	NULL	sphingomyelin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In BHK cells labeled to equilibrium with ( 3H ) choline and treated with sphingomyelinase the surface pool of sphingomyelin is degraded very rapidly ( half-time 10 min ) but the internal pool of sphingomyelin which accounts for about 30 % of the total is only degraded slowly ( half-time about 80 h ) showing that the internal pool does not normally reach the surface .
	manualset3
215626	6	419850	7	NULL	NULL	0	NULL	half-time 10 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In BHK cells labeled to equilibrium with ( 3H ) choline and treated with sphingomyelinase the surface pool of sphingomyelin is degraded very rapidly ( half-time 10 min ) but the internal pool of sphingomyelin which accounts for about 30 % of the total is only degraded slowly ( half-time about 80 h ) showing that the internal pool does not normally reach the surface .
	manualset3
215627	7	419850	7	NULL	NULL	0	NULL	internal pool 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In BHK cells labeled to equilibrium with ( 3H ) choline and treated with sphingomyelinase the surface pool of sphingomyelin is degraded very rapidly ( half-time 10 min ) but the internal pool of sphingomyelin which accounts for about 30 % of the total is only degraded slowly ( half-time about 80 h ) showing that the internal pool does not normally reach the surface .
	manualset3
215628	8	419850	7	NULL	NULL	0	NULL	sphingomyelin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In BHK cells labeled to equilibrium with ( 3H ) choline and treated with sphingomyelinase the surface pool of sphingomyelin is degraded very rapidly ( half-time 10 min ) but the internal pool of sphingomyelin which accounts for about 30 % of the total is only degraded slowly ( half-time about 80 h ) showing that the internal pool does not normally reach the surface .
	manualset3
215629	9	419850	7	NULL	NULL	0	NULL	30 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In BHK cells labeled to equilibrium with ( 3H ) choline and treated with sphingomyelinase the surface pool of sphingomyelin is degraded very rapidly ( half-time 10 min ) but the internal pool of sphingomyelin which accounts for about 30 % of the total is only degraded slowly ( half-time about 80 h ) showing that the internal pool does not normally reach the surface .
	manualset3
215630	10	419850	7	NULL	NULL	0	NULL	 total	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In BHK cells labeled to equilibrium with ( 3H ) choline and treated with sphingomyelinase the surface pool of sphingomyelin is degraded very rapidly ( half-time 10 min ) but the internal pool of sphingomyelin which accounts for about 30 % of the total is only degraded slowly ( half-time about 80 h ) showing that the internal pool does not normally reach the surface .
	manualset3
215631	11	419850	7	NULL	NULL	0	NULL	 half-time about 80 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In BHK cells labeled to equilibrium with ( 3H ) choline and treated with sphingomyelinase the surface pool of sphingomyelin is degraded very rapidly ( half-time 10 min ) but the internal pool of sphingomyelin which accounts for about 30 % of the total is only degraded slowly ( half-time about 80 h ) showing that the internal pool does not normally reach the surface .
	manualset3
215632	12	419850	7	NULL	NULL	0	NULL	 internal pool	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In BHK cells labeled to equilibrium with ( 3H ) choline and treated with sphingomyelinase the surface pool of sphingomyelin is degraded very rapidly ( half-time 10 min ) but the internal pool of sphingomyelin which accounts for about 30 % of the total is only degraded slowly ( half-time about 80 h ) showing that the internal pool does not normally reach the surface .
	manualset3
215633	13	419850	7	NULL	NULL	0	NULL	surface	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In BHK cells labeled to equilibrium with ( 3H ) choline and treated with sphingomyelinase the surface pool of sphingomyelin is degraded very rapidly ( half-time 10 min ) but the internal pool of sphingomyelin which accounts for about 30 % of the total is only degraded slowly ( half-time about 80 h ) showing that the internal pool does not normally reach the surface .
	manualset3
215634	1	419851	7	NULL	NULL	0	NULL	Vancomycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Vancomycin for treatment of invasive , multi-drug resistant Staphylococcus aureus infections .
	manualset3
215635	2	419851	7	NULL	NULL	0	NULL	 treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Vancomycin for treatment of invasive , multi-drug resistant Staphylococcus aureus infections .
	manualset3
215636	3	419851	7	NULL	NULL	0	NULL	invasive , multi-drug resistant Staphylococcus aureus infections 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Vancomycin for treatment of invasive , multi-drug resistant Staphylococcus aureus infections .
	manualset3
215637	1	419852	7	NULL	NULL	0	NULL	 continuity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the continuity of the tumor BM composed of these materials was much greater in the higher metastatic LM12-3 and LM60-D6 tumors than in those with the low metastatic P29 tumor .
	manualset3
215638	2	419852	7	NULL	NULL	0	NULL	 tumor BM	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the continuity of the tumor BM composed of these materials was much greater in the higher metastatic LM12-3 and LM60-D6 tumors than in those with the low metastatic P29 tumor .
	manualset3
215639	3	419852	7	NULL	NULL	0	NULL	materials	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the continuity of the tumor BM composed of these materials was much greater in the higher metastatic LM12-3 and LM60-D6 tumors than in those with the low metastatic P29 tumor .
	manualset3
215640	4	419852	7	NULL	NULL	0	NULL	higher metastatic LM12-3 tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the continuity of the tumor BM composed of these materials was much greater in the higher metastatic LM12-3 and LM60-D6 tumors than in those with the low metastatic P29 tumor .
	manualset3
215641	5	419852	7	NULL	NULL	0	NULL	LM60-D6 tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the continuity of the tumor BM composed of these materials was much greater in the higher metastatic LM12-3 and LM60-D6 tumors than in those with the low metastatic P29 tumor .
	manualset3
215642	6	419852	7	NULL	NULL	0	NULL	 low metastatic P29 tumor 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the continuity of the tumor BM composed of these materials was much greater in the higher metastatic LM12-3 and LM60-D6 tumors than in those with the low metastatic P29 tumor .
	manualset3
215643	1	419853	7	NULL	NULL	0	NULL	100 d gestation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	At 100 d gestation ( term 145 d ) , ANP staining was absent and NPR-A staining was weak in cuboidal epithelial cells .
	manualset3
215644	2	419853	7	NULL	NULL	0	NULL	term 145 d 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	At 100 d gestation ( term 145 d ) , ANP staining was absent and NPR-A staining was weak in cuboidal epithelial cells .
	manualset3
215645	3	419853	7	NULL	NULL	0	NULL	ANP staining	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	At 100 d gestation ( term 145 d ) , ANP staining was absent and NPR-A staining was weak in cuboidal epithelial cells .
	manualset3
215646	4	419853	7	NULL	NULL	0	NULL	NPR-A staining	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	At 100 d gestation ( term 145 d ) , ANP staining was absent and NPR-A staining was weak in cuboidal epithelial cells .
	manualset3
215647	5	419853	7	NULL	NULL	0	NULL	cuboidal epithelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	At 100 d gestation ( term 145 d ) , ANP staining was absent and NPR-A staining was weak in cuboidal epithelial cells .
	manualset3
215648	1	419854	7	NULL	NULL	0	NULL	acid-induced GMBF response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the acid-induced GMBF and DAS responses were significantly mitigated by both indomethacin and sensory deafferentation but not by ruthenium red ( RT ) , the vanilloid receptor ( VR ) -1 antagonist , the responses were preserved in lafutidine-treated animals , even in the presence of indomethacin .
	manualset3
215649	2	419854	7	NULL	NULL	0	NULL	DAS responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the acid-induced GMBF and DAS responses were significantly mitigated by both indomethacin and sensory deafferentation but not by ruthenium red ( RT ) , the vanilloid receptor ( VR ) -1 antagonist , the responses were preserved in lafutidine-treated animals , even in the presence of indomethacin .
	manualset3
215650	3	419854	7	NULL	NULL	0	NULL	 indomethacin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the acid-induced GMBF and DAS responses were significantly mitigated by both indomethacin and sensory deafferentation but not by ruthenium red ( RT ) , the vanilloid receptor ( VR ) -1 antagonist , the responses were preserved in lafutidine-treated animals , even in the presence of indomethacin .
	manualset3
215651	4	419854	7	NULL	NULL	0	NULL	sensory deafferentation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the acid-induced GMBF and DAS responses were significantly mitigated by both indomethacin and sensory deafferentation but not by ruthenium red ( RT ) , the vanilloid receptor ( VR ) -1 antagonist , the responses were preserved in lafutidine-treated animals , even in the presence of indomethacin .
	manualset3
215652	5	419854	7	NULL	NULL	0	NULL	ruthenium red ( RT ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the acid-induced GMBF and DAS responses were significantly mitigated by both indomethacin and sensory deafferentation but not by ruthenium red ( RT ) , the vanilloid receptor ( VR ) -1 antagonist , the responses were preserved in lafutidine-treated animals , even in the presence of indomethacin .
	manualset3
215653	6	419854	7	NULL	NULL	0	NULL	vanilloid receptor ( VR ) -1 antagonist 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the acid-induced GMBF and DAS responses were significantly mitigated by both indomethacin and sensory deafferentation but not by ruthenium red ( RT ) , the vanilloid receptor ( VR ) -1 antagonist , the responses were preserved in lafutidine-treated animals , even in the presence of indomethacin .
	manualset3
215654	7	419854	7	NULL	NULL	0	NULL	 responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the acid-induced GMBF and DAS responses were significantly mitigated by both indomethacin and sensory deafferentation but not by ruthenium red ( RT ) , the vanilloid receptor ( VR ) -1 antagonist , the responses were preserved in lafutidine-treated animals , even in the presence of indomethacin .
	manualset3
215655	8	419854	7	NULL	NULL	0	NULL	lafutidine-treated animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the acid-induced GMBF and DAS responses were significantly mitigated by both indomethacin and sensory deafferentation but not by ruthenium red ( RT ) , the vanilloid receptor ( VR ) -1 antagonist , the responses were preserved in lafutidine-treated animals , even in the presence of indomethacin .
	manualset3
215656	9	419854	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the acid-induced GMBF and DAS responses were significantly mitigated by both indomethacin and sensory deafferentation but not by ruthenium red ( RT ) , the vanilloid receptor ( VR ) -1 antagonist , the responses were preserved in lafutidine-treated animals , even in the presence of indomethacin .
	manualset3
215657	10	419854	7	NULL	NULL	0	NULL	indomethacin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the acid-induced GMBF and DAS responses were significantly mitigated by both indomethacin and sensory deafferentation but not by ruthenium red ( RT ) , the vanilloid receptor ( VR ) -1 antagonist , the responses were preserved in lafutidine-treated animals , even in the presence of indomethacin .
	manualset3
215658	1	419855	7	NULL	NULL	0	NULL	Integrated management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrated management of chronic pain .
	manualset3
215659	2	419855	7	NULL	NULL	0	NULL	chronic pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Integrated management of chronic pain .
	manualset3
215660	1	419856	7	NULL	NULL	0	NULL	high-resolution ex situ AFM images	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The high-resolution ex situ AFM and STM images showed that some fibrils of beta-amyloid had a characteristic domain texture , indicating they were formed through the association of protofibrils and monomers .
	manualset3
215661	2	419856	7	NULL	NULL	0	NULL	high-resolution ex situ STM images	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The high-resolution ex situ AFM and STM images showed that some fibrils of beta-amyloid had a characteristic domain texture , indicating they were formed through the association of protofibrils and monomers .
	manualset3
215662	3	419856	7	NULL	NULL	NULL	NULL	fibrils of beta-amyloid	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The high-resolution ex situ AFM and STM images showed that some fibrils of beta-amyloid had a characteristic domain texture , indicating they were formed through the association of protofibrils and monomers .
	manualset3
215663	4	419856	7	NULL	NULL	0	NULL	domain texture	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The high-resolution ex situ AFM and STM images showed that some fibrils of beta-amyloid had a characteristic domain texture , indicating they were formed through the association of protofibrils and monomers .
	manualset3
215664	5	419856	7	NULL	NULL	0	NULL	association	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The high-resolution ex situ AFM and STM images showed that some fibrils of beta-amyloid had a characteristic domain texture , indicating they were formed through the association of protofibrils and monomers .
	manualset3
215665	6	419856	7	NULL	NULL	0	NULL	protofibrils	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The high-resolution ex situ AFM and STM images showed that some fibrils of beta-amyloid had a characteristic domain texture , indicating they were formed through the association of protofibrils and monomers .
	manualset3
215666	7	419856	7	NULL	NULL	0	NULL	monomers	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The high-resolution ex situ AFM and STM images showed that some fibrils of beta-amyloid had a characteristic domain texture , indicating they were formed through the association of protofibrils and monomers .
	manualset3
215667	1	419857	7	NULL	NULL	0	NULL	Adenoviral interleukin-12 gene transduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenoviral interleukin-12 gene transduction into human bronchial epithelial cells : up-regulation of pro-inflammatory cytokines and its prevention by corticosteroids .
	manualset3
215668	2	419857	7	NULL	NULL	0	NULL	human bronchial epithelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenoviral interleukin-12 gene transduction into human bronchial epithelial cells : up-regulation of pro-inflammatory cytokines and its prevention by corticosteroids .
	manualset3
215669	3	419857	7	NULL	NULL	0	NULL	up-regulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenoviral interleukin-12 gene transduction into human bronchial epithelial cells : up-regulation of pro-inflammatory cytokines and its prevention by corticosteroids .
	manualset3
215670	4	419857	7	NULL	NULL	0	NULL	pro-inflammatory cytokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenoviral interleukin-12 gene transduction into human bronchial epithelial cells : up-regulation of pro-inflammatory cytokines and its prevention by corticosteroids .
	manualset3
215671	5	419857	7	NULL	NULL	0	NULL	prevention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenoviral interleukin-12 gene transduction into human bronchial epithelial cells : up-regulation of pro-inflammatory cytokines and its prevention by corticosteroids .
	manualset3
215672	6	419857	7	NULL	NULL	0	NULL	corticosteroids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenoviral interleukin-12 gene transduction into human bronchial epithelial cells : up-regulation of pro-inflammatory cytokines and its prevention by corticosteroids .
	manualset3
215673	1	419858	7	NULL	NULL	0	NULL	rare case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The rare case of isolated tuberculosis of the larynx in 19-year old patient was presented in this paper .
	manualset3
215674	2	419858	7	NULL	NULL	0	NULL	 isolated tuberculosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The rare case of isolated tuberculosis of the larynx in 19-year old patient was presented in this paper .
	manualset3
215675	3	419858	7	NULL	NULL	0	NULL	larynx	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The rare case of isolated tuberculosis of the larynx in 19-year old patient was presented in this paper .
	manualset3
215676	4	419858	7	NULL	NULL	0	NULL	19-year old patient	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The rare case of isolated tuberculosis of the larynx in 19-year old patient was presented in this paper .
	manualset3
215677	5	419858	7	NULL	NULL	0	NULL	paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The rare case of isolated tuberculosis of the larynx in 19-year old patient was presented in this paper .
	manualset3
215678	1	419859	7	NULL	NULL	0	NULL	redox potential	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we have shown that the redox potential of this disulfide bond is approximately -190 mV , a high value for a disulfide bond in proteins .
	manualset3
215679	2	419859	7	NULL	NULL	0	NULL	disulfide bond 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we have shown that the redox potential of this disulfide bond is approximately -190 mV , a high value for a disulfide bond in proteins .
	manualset3
215680	3	419859	7	NULL	NULL	0	NULL	-190 mV	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we have shown that the redox potential of this disulfide bond is approximately -190 mV , a high value for a disulfide bond in proteins .
	manualset3
215681	4	419859	7	NULL	NULL	0	NULL	 high value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we have shown that the redox potential of this disulfide bond is approximately -190 mV , a high value for a disulfide bond in proteins .
	manualset3
215682	5	419859	7	NULL	NULL	0	NULL	 disulfide bond 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we have shown that the redox potential of this disulfide bond is approximately -190 mV , a high value for a disulfide bond in proteins .
	manualset3
215683	6	419859	7	NULL	NULL	0	NULL	proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we have shown that the redox potential of this disulfide bond is approximately -190 mV , a high value for a disulfide bond in proteins .
	manualset3
215684	1	419860	7	NULL	NULL	0	NULL	 addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the addition of laropiprant will reduce the frequency of flushing , it will not completely eliminate this side effect .
	manualset3
215685	2	419860	7	NULL	NULL	0	NULL	 laropiprant	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the addition of laropiprant will reduce the frequency of flushing , it will not completely eliminate this side effect .
	manualset3
215686	3	419860	7	NULL	NULL	0	NULL	frequency 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the addition of laropiprant will reduce the frequency of flushing , it will not completely eliminate this side effect .
	manualset3
215687	4	419860	7	NULL	NULL	0	NULL	flushing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the addition of laropiprant will reduce the frequency of flushing , it will not completely eliminate this side effect .
	manualset3
215688	5	419860	7	NULL	NULL	0	NULL	side effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the addition of laropiprant will reduce the frequency of flushing , it will not completely eliminate this side effect .
	manualset3
215689	1	419861	7	NULL	NULL	0	NULL	Cardiac electrophysiological phenotypes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Cardiac electrophysiological phenotypes in postnatal expression of Nkx2 .5 transgenic mice .
	manualset3
215690	2	419861	7	NULL	NULL	0	NULL	postnatal expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cardiac electrophysiological phenotypes in postnatal expression of Nkx2 .5 transgenic mice .
	manualset3
215691	3	419861	7	NULL	NULL	0	NULL	Nkx2 .5 transgenic mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Cardiac electrophysiological phenotypes in postnatal expression of Nkx2 .5 transgenic mice .
	manualset3
215692	1	419862	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article is part of a Special Issue entitled Protein translocation across or insertion into membranes .
	manualset3
215693	2	419862	7	NULL	NULL	0	NULL	Special Issue	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article is part of a Special Issue entitled Protein translocation across or insertion into membranes .
	manualset3
215694	3	419862	7	NULL	NULL	0	NULL	Protein translocation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This article is part of a Special Issue entitled Protein translocation across or insertion into membranes .
	manualset3
215695	4	419862	7	NULL	NULL	0	NULL	insertion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This article is part of a Special Issue entitled Protein translocation across or insertion into membranes .
	manualset3
215696	5	419862	7	NULL	NULL	0	NULL	membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	This article is part of a Special Issue entitled Protein translocation across or insertion into membranes .
	manualset3
215697	1	419863	7	NULL	NULL	0	NULL	 role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role played by hippocampal mossy fibers in the learning and memory processes implemented in the Morris swimming navigation task has been studied in C57BL/6 mice by selective and reversible inactivation of mossy fiber synaptic fields by diethyldithiocarbamate .
	manualset3
215698	2	419863	7	NULL	NULL	0	NULL	hippocampal mossy fibers	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The role played by hippocampal mossy fibers in the learning and memory processes implemented in the Morris swimming navigation task has been studied in C57BL/6 mice by selective and reversible inactivation of mossy fiber synaptic fields by diethyldithiocarbamate .
	manualset3
215699	3	419863	7	NULL	NULL	0	NULL	 learning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role played by hippocampal mossy fibers in the learning and memory processes implemented in the Morris swimming navigation task has been studied in C57BL/6 mice by selective and reversible inactivation of mossy fiber synaptic fields by diethyldithiocarbamate .
	manualset3
215700	4	419863	7	NULL	NULL	0	NULL	memory processes	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role played by hippocampal mossy fibers in the learning and memory processes implemented in the Morris swimming navigation task has been studied in C57BL/6 mice by selective and reversible inactivation of mossy fiber synaptic fields by diethyldithiocarbamate .
	manualset3
215701	5	419863	7	NULL	NULL	0	NULL	Morris swimming navigation task	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The role played by hippocampal mossy fibers in the learning and memory processes implemented in the Morris swimming navigation task has been studied in C57BL/6 mice by selective and reversible inactivation of mossy fiber synaptic fields by diethyldithiocarbamate .
	manualset3
215702	6	419863	7	NULL	NULL	0	NULL	C57BL/6 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The role played by hippocampal mossy fibers in the learning and memory processes implemented in the Morris swimming navigation task has been studied in C57BL/6 mice by selective and reversible inactivation of mossy fiber synaptic fields by diethyldithiocarbamate .
	manualset3
215703	7	419863	7	NULL	NULL	0	NULL	selective and reversible inactivation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role played by hippocampal mossy fibers in the learning and memory processes implemented in the Morris swimming navigation task has been studied in C57BL/6 mice by selective and reversible inactivation of mossy fiber synaptic fields by diethyldithiocarbamate .
	manualset3
215704	8	419863	7	NULL	NULL	0	NULL	 mossy fiber synaptic fields	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The role played by hippocampal mossy fibers in the learning and memory processes implemented in the Morris swimming navigation task has been studied in C57BL/6 mice by selective and reversible inactivation of mossy fiber synaptic fields by diethyldithiocarbamate .
	manualset3
215705	9	419863	7	NULL	NULL	0	NULL	diethyldithiocarbamate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The role played by hippocampal mossy fibers in the learning and memory processes implemented in the Morris swimming navigation task has been studied in C57BL/6 mice by selective and reversible inactivation of mossy fiber synaptic fields by diethyldithiocarbamate .
	manualset3
215706	1	419864	7	NULL	NULL	0	NULL	Pretreatment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of animals with enalaprilat prior to sham operation prevented the increase in glomerular eicosanoid production and cyclooxygenase content in SOC rats fed a high-protein diet and the levels observed were similar to those in SOC rats fed a low-protein diet .
	manualset3
215707	2	419864	7	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of animals with enalaprilat prior to sham operation prevented the increase in glomerular eicosanoid production and cyclooxygenase content in SOC rats fed a high-protein diet and the levels observed were similar to those in SOC rats fed a low-protein diet .
	manualset3
215708	3	419864	7	NULL	NULL	0	NULL	enalaprilat	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of animals with enalaprilat prior to sham operation prevented the increase in glomerular eicosanoid production and cyclooxygenase content in SOC rats fed a high-protein diet and the levels observed were similar to those in SOC rats fed a low-protein diet .
	manualset3
215709	4	419864	7	NULL	NULL	0	NULL	sham operation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of animals with enalaprilat prior to sham operation prevented the increase in glomerular eicosanoid production and cyclooxygenase content in SOC rats fed a high-protein diet and the levels observed were similar to those in SOC rats fed a low-protein diet .
	manualset3
215710	5	419864	7	NULL	NULL	0	NULL	 increase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of animals with enalaprilat prior to sham operation prevented the increase in glomerular eicosanoid production and cyclooxygenase content in SOC rats fed a high-protein diet and the levels observed were similar to those in SOC rats fed a low-protein diet .
	manualset3
215711	6	419864	7	NULL	NULL	0	NULL	glomerular eicosanoid production 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of animals with enalaprilat prior to sham operation prevented the increase in glomerular eicosanoid production and cyclooxygenase content in SOC rats fed a high-protein diet and the levels observed were similar to those in SOC rats fed a low-protein diet .
	manualset3
215712	7	419864	7	NULL	NULL	0	NULL	cyclooxygenase content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of animals with enalaprilat prior to sham operation prevented the increase in glomerular eicosanoid production and cyclooxygenase content in SOC rats fed a high-protein diet and the levels observed were similar to those in SOC rats fed a low-protein diet .
	manualset3
215713	8	419864	7	NULL	NULL	0	NULL	SOC rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of animals with enalaprilat prior to sham operation prevented the increase in glomerular eicosanoid production and cyclooxygenase content in SOC rats fed a high-protein diet and the levels observed were similar to those in SOC rats fed a low-protein diet .
	manualset3
215714	9	419864	7	NULL	NULL	0	NULL	high-protein diet 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of animals with enalaprilat prior to sham operation prevented the increase in glomerular eicosanoid production and cyclooxygenase content in SOC rats fed a high-protein diet and the levels observed were similar to those in SOC rats fed a low-protein diet .
	manualset3
215715	10	419864	7	NULL	NULL	0	NULL	levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of animals with enalaprilat prior to sham operation prevented the increase in glomerular eicosanoid production and cyclooxygenase content in SOC rats fed a high-protein diet and the levels observed were similar to those in SOC rats fed a low-protein diet .
	manualset3
215716	11	419864	7	NULL	NULL	0	NULL	SOC rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of animals with enalaprilat prior to sham operation prevented the increase in glomerular eicosanoid production and cyclooxygenase content in SOC rats fed a high-protein diet and the levels observed were similar to those in SOC rats fed a low-protein diet .
	manualset3
215717	12	419864	7	NULL	NULL	0	NULL	low-protein diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment of animals with enalaprilat prior to sham operation prevented the increase in glomerular eicosanoid production and cyclooxygenase content in SOC rats fed a high-protein diet and the levels observed were similar to those in SOC rats fed a low-protein diet .
	manualset3
215718	1	419865	7	NULL	NULL	0	NULL	water fluoride level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The water fluoride level was estimated in 6 town sources twice , using Alizarin chemical method .
	manualset3
215719	2	419865	7	NULL	NULL	0	NULL	6 town sources	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The water fluoride level was estimated in 6 town sources twice , using Alizarin chemical method .
	manualset3
215720	3	419865	7	NULL	NULL	0	NULL	 Alizarin chemical method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The water fluoride level was estimated in 6 town sources twice , using Alizarin chemical method .
	manualset3
215721	1	419866	7	NULL	NULL	0	NULL	Serum chemistry	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum chemistry of bowhead whales ( Balaena mysticetus ) .
	manualset3
215722	2	419866	7	NULL	NULL	0	NULL	bowhead whales	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum chemistry of bowhead whales ( Balaena mysticetus ) .
	manualset3
215723	3	419866	7	NULL	NULL	0	NULL	Balaena mysticetus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum chemistry of bowhead whales ( Balaena mysticetus ) .
	manualset3
215724	1	419867	7	NULL	NULL	NULL	NULL	alpha-helical Y ( X ) 4Lvarphi containing region	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although the alpha-helical Y ( X ) 4Lvarphi containing region of eIF4E-binding protein ( 4EBP ) is the major binding region with eukaryotic initiation factor 4E ( eIF4E ) , the roles of its N - and C-terminal regions in the binding are hardly known .
	manualset3
215725	2	419867	7	NULL	NULL	0	NULL	eIF4E-binding protein ( 4EBP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the alpha-helical Y ( X ) 4Lvarphi containing region of eIF4E-binding protein ( 4EBP ) is the major binding region with eukaryotic initiation factor 4E ( eIF4E ) , the roles of its N - and C-terminal regions in the binding are hardly known .
	manualset3
215726	3	419867	7	NULL	NULL	0	NULL	binding region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the alpha-helical Y ( X ) 4Lvarphi containing region of eIF4E-binding protein ( 4EBP ) is the major binding region with eukaryotic initiation factor 4E ( eIF4E ) , the roles of its N - and C-terminal regions in the binding are hardly known .
	manualset3
215727	4	419867	7	NULL	NULL	0	NULL	eukaryotic initiation factor 4E ( eIF4E )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the alpha-helical Y ( X ) 4Lvarphi containing region of eIF4E-binding protein ( 4EBP ) is the major binding region with eukaryotic initiation factor 4E ( eIF4E ) , the roles of its N - and C-terminal regions in the binding are hardly known .
	manualset3
215728	5	419867	7	NULL	NULL	0	NULL	roles	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the alpha-helical Y ( X ) 4Lvarphi containing region of eIF4E-binding protein ( 4EBP ) is the major binding region with eukaryotic initiation factor 4E ( eIF4E ) , the roles of its N - and C-terminal regions in the binding are hardly known .
	manualset3
215729	6	419867	7	NULL	NULL	0	NULL	N - terminal region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the alpha-helical Y ( X ) 4Lvarphi containing region of eIF4E-binding protein ( 4EBP ) is the major binding region with eukaryotic initiation factor 4E ( eIF4E ) , the roles of its N - and C-terminal regions in the binding are hardly known .
	manualset3
215730	7	419867	7	NULL	NULL	0	NULL	C-terminal regions	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the alpha-helical Y ( X ) 4Lvarphi containing region of eIF4E-binding protein ( 4EBP ) is the major binding region with eukaryotic initiation factor 4E ( eIF4E ) , the roles of its N - and C-terminal regions in the binding are hardly known .
	manualset3
215731	8	419867	7	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the alpha-helical Y ( X ) 4Lvarphi containing region of eIF4E-binding protein ( 4EBP ) is the major binding region with eukaryotic initiation factor 4E ( eIF4E ) , the roles of its N - and C-terminal regions in the binding are hardly known .
	manualset3
215732	1	419868	7	NULL	NULL	NULL	NULL	changes	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Some changes in the antigenic complex of Bacillus anthracis under the action of streptomycin ) .
	manualset3
215733	2	419868	7	NULL	NULL	0	NULL	antigenic complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Some changes in the antigenic complex of Bacillus anthracis under the action of streptomycin ) .
	manualset3
215734	3	419868	7	NULL	NULL	0	NULL	Bacillus anthracis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Some changes in the antigenic complex of Bacillus anthracis under the action of streptomycin ) .
	manualset3
215735	4	419868	7	NULL	NULL	0	NULL	action	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Some changes in the antigenic complex of Bacillus anthracis under the action of streptomycin ) .
	manualset3
215736	5	419868	7	NULL	NULL	0	NULL	streptomycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Some changes in the antigenic complex of Bacillus anthracis under the action of streptomycin ) .
	manualset3
215737	1	419869	7	NULL	NULL	0	NULL	Acetylcholine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetylcholine leads to free radical production dependent on K ( ATP ) channels , G ( i ) proteins , phosphatidylinositol 3-kinase and tyrosine kinase .
	manualset3
215738	2	419869	7	NULL	NULL	0	NULL	free radical production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetylcholine leads to free radical production dependent on K ( ATP ) channels , G ( i ) proteins , phosphatidylinositol 3-kinase and tyrosine kinase .
	manualset3
215739	3	419869	7	NULL	NULL	0	NULL	K ( ATP ) channels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetylcholine leads to free radical production dependent on K ( ATP ) channels , G ( i ) proteins , phosphatidylinositol 3-kinase and tyrosine kinase .
	manualset3
215740	4	419869	7	NULL	NULL	0	NULL	G ( i ) proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetylcholine leads to free radical production dependent on K ( ATP ) channels , G ( i ) proteins , phosphatidylinositol 3-kinase and tyrosine kinase .
	manualset3
215741	5	419869	7	NULL	NULL	0	NULL	phosphatidylinositol 3-kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetylcholine leads to free radical production dependent on K ( ATP ) channels , G ( i ) proteins , phosphatidylinositol 3-kinase and tyrosine kinase .
	manualset3
215742	6	419869	7	NULL	NULL	0	NULL	tyrosine kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Acetylcholine leads to free radical production dependent on K ( ATP ) channels , G ( i ) proteins , phosphatidylinositol 3-kinase and tyrosine kinase .
	manualset3
215743	1	419870	7	NULL	NULL	0	NULL	Comparison	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of two different implantation processing techniques for random dopant ( RD ) - induced threshold voltage fluctuation ( sigmaV ( th ) ) in 15-nm metal-oxide-semiconductor ( MOS ) devices is reported .
	manualset3
215744	2	419870	7	NULL	NULL	0	NULL	two different implantation processing techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of two different implantation processing techniques for random dopant ( RD ) - induced threshold voltage fluctuation ( sigmaV ( th ) ) in 15-nm metal-oxide-semiconductor ( MOS ) devices is reported .
	manualset3
215745	3	419870	7	NULL	NULL	0	NULL	random dopant ( RD ) - induced threshold voltage fluctuation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of two different implantation processing techniques for random dopant ( RD ) - induced threshold voltage fluctuation ( sigmaV ( th ) ) in 15-nm metal-oxide-semiconductor ( MOS ) devices is reported .
	manualset3
215746	4	419870	7	NULL	NULL	0	NULL	( sigmaV ( th ) )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of two different implantation processing techniques for random dopant ( RD ) - induced threshold voltage fluctuation ( sigmaV ( th ) ) in 15-nm metal-oxide-semiconductor ( MOS ) devices is reported .
	manualset3
215747	5	419870	7	NULL	NULL	NULL	NULL	15-nm metal-oxide-semiconductor devices	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Comparison of two different implantation processing techniques for random dopant ( RD ) - induced threshold voltage fluctuation ( sigmaV ( th ) ) in 15-nm metal-oxide-semiconductor ( MOS ) devices is reported .
	manualset3
215748	6	419870	7	NULL	NULL	0	NULL	( MOS ) 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of two different implantation processing techniques for random dopant ( RD ) - induced threshold voltage fluctuation ( sigmaV ( th ) ) in 15-nm metal-oxide-semiconductor ( MOS ) devices is reported .
	manualset3
215749	1	419871	7	NULL	NULL	0	NULL	SNM	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It appears that SNM produces a modulation of medullary reflexes and brain centers by peripheral afferents .
	manualset3
215750	2	419871	7	NULL	NULL	0	NULL	modulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It appears that SNM produces a modulation of medullary reflexes and brain centers by peripheral afferents .
	manualset3
215751	3	419871	7	NULL	NULL	0	NULL	medullary reflexes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It appears that SNM produces a modulation of medullary reflexes and brain centers by peripheral afferents .
	manualset3
215752	4	419871	7	NULL	NULL	0	NULL	brain centers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It appears that SNM produces a modulation of medullary reflexes and brain centers by peripheral afferents .
	manualset3
215753	5	419871	7	NULL	NULL	0	NULL	peripheral afferents	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It appears that SNM produces a modulation of medullary reflexes and brain centers by peripheral afferents .
	manualset3
215754	1	419872	7	NULL	NULL	0	NULL	Clinical phase I pharmacokinetic studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical phase I pharmacokinetic studies with lornoxicam were performed with the 4 mg dose of lornoxicam .
	manualset3
215755	2	419872	7	NULL	NULL	0	NULL	lornoxicam	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical phase I pharmacokinetic studies with lornoxicam were performed with the 4 mg dose of lornoxicam .
	manualset3
215756	3	419872	7	NULL	NULL	0	NULL	4 mg dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical phase I pharmacokinetic studies with lornoxicam were performed with the 4 mg dose of lornoxicam .
	manualset3
215757	4	419872	7	NULL	NULL	0	NULL	 lornoxicam	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical phase I pharmacokinetic studies with lornoxicam were performed with the 4 mg dose of lornoxicam .
	manualset3
215758	1	419873	7	NULL	NULL	0	NULL	 patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient was also found to have a papillary thyroid carcinoma and hypergastrinemia .
	manualset3
215759	2	419873	7	NULL	NULL	0	NULL	papillary thyroid carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient was also found to have a papillary thyroid carcinoma and hypergastrinemia .
	manualset3
215760	3	419873	7	NULL	NULL	0	NULL	hypergastrinemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient was also found to have a papillary thyroid carcinoma and hypergastrinemia .
	manualset3
215761	1	419874	7	NULL	NULL	0	NULL	 80 + Project	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The 80 + Project represents a foundation of information and offers promise to create durable , productive interactions for elderly individuals and their health care providers .
	manualset3
215762	2	419874	7	NULL	NULL	0	NULL	foundation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 80 + Project represents a foundation of information and offers promise to create durable , productive interactions for elderly individuals and their health care providers .
	manualset3
215763	3	419874	7	NULL	NULL	0	NULL	 information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The 80 + Project represents a foundation of information and offers promise to create durable , productive interactions for elderly individuals and their health care providers .
	manualset3
215764	4	419874	7	NULL	NULL	0	NULL	productive interactions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 80 + Project represents a foundation of information and offers promise to create durable , productive interactions for elderly individuals and their health care providers .
	manualset3
215765	5	419874	7	NULL	NULL	0	NULL	 elderly individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The 80 + Project represents a foundation of information and offers promise to create durable , productive interactions for elderly individuals and their health care providers .
	manualset3
215766	6	419874	7	NULL	NULL	0	NULL	health care providers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The 80 + Project represents a foundation of information and offers promise to create durable , productive interactions for elderly individuals and their health care providers .
	manualset3
215767	1	419875	7	NULL	NULL	0	NULL	Product sampling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Product sampling -- why bother ?
	manualset3
215768	1	419876	7	NULL	NULL	0	NULL	DSM IV criteria	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( DSM IV criteria for post-partum depression : debatable ? ) .
	manualset3
215769	2	419876	7	NULL	NULL	0	NULL	post-partum depression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( DSM IV criteria for post-partum depression : debatable ? ) .
	manualset3
215770	1	419877	7	NULL	NULL	0	NULL	amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the amount of apoptosis was of the same order of magnitude at its peak ( 24 h ) at both doses , only 400 mg/kg 5-FU brought about histopathological changes to the gut after 96 h , quantified as losses of crypt and villus cellularity .
	manualset3
215771	2	419877	7	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the amount of apoptosis was of the same order of magnitude at its peak ( 24 h ) at both doses , only 400 mg/kg 5-FU brought about histopathological changes to the gut after 96 h , quantified as losses of crypt and villus cellularity .
	manualset3
215772	3	419877	7	NULL	NULL	0	NULL	order of magnitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the amount of apoptosis was of the same order of magnitude at its peak ( 24 h ) at both doses , only 400 mg/kg 5-FU brought about histopathological changes to the gut after 96 h , quantified as losses of crypt and villus cellularity .
	manualset3
215773	4	419877	7	NULL	NULL	0	NULL	peak 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the amount of apoptosis was of the same order of magnitude at its peak ( 24 h ) at both doses , only 400 mg/kg 5-FU brought about histopathological changes to the gut after 96 h , quantified as losses of crypt and villus cellularity .
	manualset3
215774	5	419877	7	NULL	NULL	0	NULL	24 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the amount of apoptosis was of the same order of magnitude at its peak ( 24 h ) at both doses , only 400 mg/kg 5-FU brought about histopathological changes to the gut after 96 h , quantified as losses of crypt and villus cellularity .
	manualset3
215775	6	419877	7	NULL	NULL	0	NULL	doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the amount of apoptosis was of the same order of magnitude at its peak ( 24 h ) at both doses , only 400 mg/kg 5-FU brought about histopathological changes to the gut after 96 h , quantified as losses of crypt and villus cellularity .
	manualset3
215776	7	419877	7	NULL	NULL	0	NULL	400 mg/kg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the amount of apoptosis was of the same order of magnitude at its peak ( 24 h ) at both doses , only 400 mg/kg 5-FU brought about histopathological changes to the gut after 96 h , quantified as losses of crypt and villus cellularity .
	manualset3
215777	8	419877	7	NULL	NULL	0	NULL	5-FU	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the amount of apoptosis was of the same order of magnitude at its peak ( 24 h ) at both doses , only 400 mg/kg 5-FU brought about histopathological changes to the gut after 96 h , quantified as losses of crypt and villus cellularity .
	manualset3
215778	9	419877	7	NULL	NULL	0	NULL	histopathological changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the amount of apoptosis was of the same order of magnitude at its peak ( 24 h ) at both doses , only 400 mg/kg 5-FU brought about histopathological changes to the gut after 96 h , quantified as losses of crypt and villus cellularity .
	manualset3
215779	10	419877	7	NULL	NULL	0	NULL	gut	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the amount of apoptosis was of the same order of magnitude at its peak ( 24 h ) at both doses , only 400 mg/kg 5-FU brought about histopathological changes to the gut after 96 h , quantified as losses of crypt and villus cellularity .
	manualset3
215780	11	419877	7	NULL	NULL	0	NULL	96 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the amount of apoptosis was of the same order of magnitude at its peak ( 24 h ) at both doses , only 400 mg/kg 5-FU brought about histopathological changes to the gut after 96 h , quantified as losses of crypt and villus cellularity .
	manualset3
215781	12	419877	7	NULL	NULL	0	NULL	 losses of crypt cellularity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the amount of apoptosis was of the same order of magnitude at its peak ( 24 h ) at both doses , only 400 mg/kg 5-FU brought about histopathological changes to the gut after 96 h , quantified as losses of crypt and villus cellularity .
	manualset3
215782	13	419877	7	NULL	NULL	NULL	NULL	losses of villus cellularity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although the amount of apoptosis was of the same order of magnitude at its peak ( 24 h ) at both doses , only 400 mg/kg 5-FU brought about histopathological changes to the gut after 96 h , quantified as losses of crypt and villus cellularity .
	manualset3
215783	1	419878	7	NULL	NULL	0	NULL	Model-free analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Model-free analysis of ( 15 ) N relaxation parameters , T ( 1 ) , T ( 2 ) ( T ( 1rho ) ) and ( 15 ) N - ( ( 1 ) H ) NOE , shows that residues in the flap tips are flexible on the sub-ns time scale , in contrast with previous observations on the inhibitor-bound protease .
	manualset3
215784	2	419878	7	NULL	NULL	0	NULL	( 15 ) N relaxation parameters	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Model-free analysis of ( 15 ) N relaxation parameters , T ( 1 ) , T ( 2 ) ( T ( 1rho ) ) and ( 15 ) N - ( ( 1 ) H ) NOE , shows that residues in the flap tips are flexible on the sub-ns time scale , in contrast with previous observations on the inhibitor-bound protease .
	manualset3
215785	3	419878	7	NULL	NULL	0	NULL	 T ( 1 ) , T ( 2 ) ( T ( 1rho ) ) 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Model-free analysis of ( 15 ) N relaxation parameters , T ( 1 ) , T ( 2 ) ( T ( 1rho ) ) and ( 15 ) N - ( ( 1 ) H ) NOE , shows that residues in the flap tips are flexible on the sub-ns time scale , in contrast with previous observations on the inhibitor-bound protease .
	manualset3
215786	4	419878	7	NULL	NULL	0	NULL	( 15 ) N - ( ( 1 ) H ) NOE 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Model-free analysis of ( 15 ) N relaxation parameters , T ( 1 ) , T ( 2 ) ( T ( 1rho ) ) and ( 15 ) N - ( ( 1 ) H ) NOE , shows that residues in the flap tips are flexible on the sub-ns time scale , in contrast with previous observations on the inhibitor-bound protease .
	manualset3
215787	5	419878	7	NULL	NULL	0	NULL	residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Model-free analysis of ( 15 ) N relaxation parameters , T ( 1 ) , T ( 2 ) ( T ( 1rho ) ) and ( 15 ) N - ( ( 1 ) H ) NOE , shows that residues in the flap tips are flexible on the sub-ns time scale , in contrast with previous observations on the inhibitor-bound protease .
	manualset3
215788	6	419878	7	NULL	NULL	0	NULL	 flap tips	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Model-free analysis of ( 15 ) N relaxation parameters , T ( 1 ) , T ( 2 ) ( T ( 1rho ) ) and ( 15 ) N - ( ( 1 ) H ) NOE , shows that residues in the flap tips are flexible on the sub-ns time scale , in contrast with previous observations on the inhibitor-bound protease .
	manualset3
215789	7	419878	7	NULL	NULL	0	NULL	 flexible	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Model-free analysis of ( 15 ) N relaxation parameters , T ( 1 ) , T ( 2 ) ( T ( 1rho ) ) and ( 15 ) N - ( ( 1 ) H ) NOE , shows that residues in the flap tips are flexible on the sub-ns time scale , in contrast with previous observations on the inhibitor-bound protease .
	manualset3
215790	8	419878	7	NULL	NULL	0	NULL	sub-ns time scale	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Model-free analysis of ( 15 ) N relaxation parameters , T ( 1 ) , T ( 2 ) ( T ( 1rho ) ) and ( 15 ) N - ( ( 1 ) H ) NOE , shows that residues in the flap tips are flexible on the sub-ns time scale , in contrast with previous observations on the inhibitor-bound protease .
	manualset3
215791	9	419878	7	NULL	NULL	0	NULL	previous observations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Model-free analysis of ( 15 ) N relaxation parameters , T ( 1 ) , T ( 2 ) ( T ( 1rho ) ) and ( 15 ) N - ( ( 1 ) H ) NOE , shows that residues in the flap tips are flexible on the sub-ns time scale , in contrast with previous observations on the inhibitor-bound protease .
	manualset3
215792	10	419878	7	NULL	NULL	0	NULL	inhibitor-bound protease	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Model-free analysis of ( 15 ) N relaxation parameters , T ( 1 ) , T ( 2 ) ( T ( 1rho ) ) and ( 15 ) N - ( ( 1 ) H ) NOE , shows that residues in the flap tips are flexible on the sub-ns time scale , in contrast with previous observations on the inhibitor-bound protease .
	manualset3
215793	1	419879	7	NULL	NULL	0	NULL	case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of recurrent meningitis due to a congenital stapes footplate defect is reported .
	manualset3
215794	2	419879	7	NULL	NULL	0	NULL	recurrent meningitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of recurrent meningitis due to a congenital stapes footplate defect is reported .
	manualset3
215795	3	419879	7	NULL	NULL	0	NULL	congenital stapes footplate defect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of recurrent meningitis due to a congenital stapes footplate defect is reported .
	manualset3
215796	1	419880	7	NULL	NULL	0	NULL	1 patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Only 1 of the 7 patients who had previously undergone endoscopic sphincterotomy for concomitant choledocholithiasis was free of stones after 1 yr of dissolution .
	manualset3
215797	2	419880	7	NULL	NULL	0	NULL	7 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Only 1 of the 7 patients who had previously undergone endoscopic sphincterotomy for concomitant choledocholithiasis was free of stones after 1 yr of dissolution .
	manualset3
215798	3	419880	7	NULL	NULL	0	NULL	endoscopic sphincterotomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Only 1 of the 7 patients who had previously undergone endoscopic sphincterotomy for concomitant choledocholithiasis was free of stones after 1 yr of dissolution .
	manualset3
215799	4	419880	7	NULL	NULL	0	NULL	concomitant choledocholithiasis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Only 1 of the 7 patients who had previously undergone endoscopic sphincterotomy for concomitant choledocholithiasis was free of stones after 1 yr of dissolution .
	manualset3
215800	5	419880	7	NULL	NULL	0	NULL	free of stones	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Only 1 of the 7 patients who had previously undergone endoscopic sphincterotomy for concomitant choledocholithiasis was free of stones after 1 yr of dissolution .
	manualset3
215801	6	419880	7	NULL	NULL	0	NULL	1 yr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Only 1 of the 7 patients who had previously undergone endoscopic sphincterotomy for concomitant choledocholithiasis was free of stones after 1 yr of dissolution .
	manualset3
215802	7	419880	7	NULL	NULL	0	NULL	dissolution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Only 1 of the 7 patients who had previously undergone endoscopic sphincterotomy for concomitant choledocholithiasis was free of stones after 1 yr of dissolution .
	manualset3
215803	1	419881	7	NULL	NULL	0	NULL	 two residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Because these two residues were proposed to form a part of the local anesthetic binding site , we conclude that amitriptyline and local anesthetics interact with a common binding site .
	manualset3
215804	2	419881	7	NULL	NULL	0	NULL	part of the local anesthetic binding site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Because these two residues were proposed to form a part of the local anesthetic binding site , we conclude that amitriptyline and local anesthetics interact with a common binding site .
	manualset3
215805	3	419881	7	NULL	NULL	0	NULL	 amitriptyline	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Because these two residues were proposed to form a part of the local anesthetic binding site , we conclude that amitriptyline and local anesthetics interact with a common binding site .
	manualset3
215806	4	419881	7	NULL	NULL	0	NULL	local anesthetics 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Because these two residues were proposed to form a part of the local anesthetic binding site , we conclude that amitriptyline and local anesthetics interact with a common binding site .
	manualset3
215807	5	419881	7	NULL	NULL	0	NULL	common binding site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Because these two residues were proposed to form a part of the local anesthetic binding site , we conclude that amitriptyline and local anesthetics interact with a common binding site .
	manualset3
215808	1	419882	7	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the association between WS and CSS that was observed in our patient may be purely coincidental , it could also suggest a common pathogenetic background of these two distinct diseases , as both share several many common features .
	manualset3
215809	2	419882	7	NULL	NULL	0	NULL	 WS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the association between WS and CSS that was observed in our patient may be purely coincidental , it could also suggest a common pathogenetic background of these two distinct diseases , as both share several many common features .
	manualset3
215810	3	419882	7	NULL	NULL	0	NULL	CSS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the association between WS and CSS that was observed in our patient may be purely coincidental , it could also suggest a common pathogenetic background of these two distinct diseases , as both share several many common features .
	manualset3
215811	4	419882	7	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the association between WS and CSS that was observed in our patient may be purely coincidental , it could also suggest a common pathogenetic background of these two distinct diseases , as both share several many common features .
	manualset3
215812	5	419882	7	NULL	NULL	0	NULL	pathogenetic background	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the association between WS and CSS that was observed in our patient may be purely coincidental , it could also suggest a common pathogenetic background of these two distinct diseases , as both share several many common features .
	manualset3
215813	6	419882	7	NULL	NULL	0	NULL	diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the association between WS and CSS that was observed in our patient may be purely coincidental , it could also suggest a common pathogenetic background of these two distinct diseases , as both share several many common features .
	manualset3
215814	7	419882	7	NULL	NULL	0	NULL	common features	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the association between WS and CSS that was observed in our patient may be purely coincidental , it could also suggest a common pathogenetic background of these two distinct diseases , as both share several many common features .
	manualset3
215815	1	419883	7	NULL	NULL	0	NULL	Voltammetric studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Voltammetric and spectroscopic studies on methyl green and cationic lipid bound to calf thymus DNA .
	manualset3
215816	2	419883	7	NULL	NULL	0	NULL	spectroscopic studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Voltammetric and spectroscopic studies on methyl green and cationic lipid bound to calf thymus DNA .
	manualset3
215817	3	419883	7	NULL	NULL	0	NULL	methyl green	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Voltammetric and spectroscopic studies on methyl green and cationic lipid bound to calf thymus DNA .
	manualset3
215818	4	419883	7	NULL	NULL	0	NULL	cationic lipid	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Voltammetric and spectroscopic studies on methyl green and cationic lipid bound to calf thymus DNA .
	manualset3
215819	5	419883	7	NULL	NULL	0	NULL	calf thymus DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Voltammetric and spectroscopic studies on methyl green and cationic lipid bound to calf thymus DNA .
	manualset3
215820	1	419884	7	NULL	NULL	0	NULL	Discal cyst	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Discal cyst of the lumbar spine : MR imaging features .
	manualset3
215821	2	419884	7	NULL	NULL	0	NULL	lumbar spine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Discal cyst of the lumbar spine : MR imaging features .
	manualset3
215822	3	419884	7	NULL	NULL	0	NULL	MR imaging features	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Discal cyst of the lumbar spine : MR imaging features .
	manualset3
215823	1	419885	7	NULL	NULL	0	NULL	Ongoing dissociation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ongoing dissociation makes bound drug available for transvascular exchange and thereby diminishes the pharmacokinetic significance of binding data obtained in vitro .
	manualset3
215824	2	419885	7	NULL	NULL	0	NULL	bound drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Ongoing dissociation makes bound drug available for transvascular exchange and thereby diminishes the pharmacokinetic significance of binding data obtained in vitro .
	manualset3
215825	3	419885	7	NULL	NULL	0	NULL	 transvascular exchange	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ongoing dissociation makes bound drug available for transvascular exchange and thereby diminishes the pharmacokinetic significance of binding data obtained in vitro .
	manualset3
215826	4	419885	7	NULL	NULL	0	NULL	pharmacokinetic significance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ongoing dissociation makes bound drug available for transvascular exchange and thereby diminishes the pharmacokinetic significance of binding data obtained in vitro .
	manualset3
215827	5	419885	7	NULL	NULL	0	NULL	binding data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Ongoing dissociation makes bound drug available for transvascular exchange and thereby diminishes the pharmacokinetic significance of binding data obtained in vitro .
	manualset3
215828	1	419886	7	NULL	NULL	0	NULL	Evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluation of the epitope specificity of anti-factor VIII antibodies in plasma samples obtained at different time-points of inhibitor development revealed initial development of a low titer inhibitor directed towards the A2 domain and factor VIII light chain .
	manualset3
215829	2	419886	7	NULL	NULL	0	NULL	epitope specificity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluation of the epitope specificity of anti-factor VIII antibodies in plasma samples obtained at different time-points of inhibitor development revealed initial development of a low titer inhibitor directed towards the A2 domain and factor VIII light chain .
	manualset3
215830	3	419886	7	NULL	NULL	0	NULL	anti-factor VIII antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluation of the epitope specificity of anti-factor VIII antibodies in plasma samples obtained at different time-points of inhibitor development revealed initial development of a low titer inhibitor directed towards the A2 domain and factor VIII light chain .
	manualset3
215831	4	419886	7	NULL	NULL	0	NULL	plasma samples	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluation of the epitope specificity of anti-factor VIII antibodies in plasma samples obtained at different time-points of inhibitor development revealed initial development of a low titer inhibitor directed towards the A2 domain and factor VIII light chain .
	manualset3
215832	5	419886	7	NULL	NULL	0	NULL	different time-points	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluation of the epitope specificity of anti-factor VIII antibodies in plasma samples obtained at different time-points of inhibitor development revealed initial development of a low titer inhibitor directed towards the A2 domain and factor VIII light chain .
	manualset3
215833	6	419886	7	NULL	NULL	0	NULL	inhibitor development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluation of the epitope specificity of anti-factor VIII antibodies in plasma samples obtained at different time-points of inhibitor development revealed initial development of a low titer inhibitor directed towards the A2 domain and factor VIII light chain .
	manualset3
215834	7	419886	7	NULL	NULL	0	NULL	initial development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluation of the epitope specificity of anti-factor VIII antibodies in plasma samples obtained at different time-points of inhibitor development revealed initial development of a low titer inhibitor directed towards the A2 domain and factor VIII light chain .
	manualset3
215835	8	419886	7	NULL	NULL	0	NULL	low titer inhibitor	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluation of the epitope specificity of anti-factor VIII antibodies in plasma samples obtained at different time-points of inhibitor development revealed initial development of a low titer inhibitor directed towards the A2 domain and factor VIII light chain .
	manualset3
215836	9	419886	7	NULL	NULL	0	NULL	A2 domain 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluation of the epitope specificity of anti-factor VIII antibodies in plasma samples obtained at different time-points of inhibitor development revealed initial development of a low titer inhibitor directed towards the A2 domain and factor VIII light chain .
	manualset3
215837	10	419886	7	NULL	NULL	0	NULL	factor VIII light chain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluation of the epitope specificity of anti-factor VIII antibodies in plasma samples obtained at different time-points of inhibitor development revealed initial development of a low titer inhibitor directed towards the A2 domain and factor VIII light chain .
	manualset3
215838	1	419887	7	NULL	NULL	0	NULL	 three experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In three experiments , participants were exposed to either alcohol or control beverage images , then asked to type as quickly as possible the first word that came to mind in response to a series of provocative ( e.g. , feces ) and neutral ( e.g. , chair ) stimulus words .
	manualset3
215839	2	419887	7	NULL	NULL	0	NULL	 participants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In three experiments , participants were exposed to either alcohol or control beverage images , then asked to type as quickly as possible the first word that came to mind in response to a series of provocative ( e.g. , feces ) and neutral ( e.g. , chair ) stimulus words .
	manualset3
215840	3	419887	7	NULL	NULL	0	NULL	alcohol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In three experiments , participants were exposed to either alcohol or control beverage images , then asked to type as quickly as possible the first word that came to mind in response to a series of provocative ( e.g. , feces ) and neutral ( e.g. , chair ) stimulus words .
	manualset3
215841	4	419887	7	NULL	NULL	0	NULL	control beverage images	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In three experiments , participants were exposed to either alcohol or control beverage images , then asked to type as quickly as possible the first word that came to mind in response to a series of provocative ( e.g. , feces ) and neutral ( e.g. , chair ) stimulus words .
	manualset3
215842	5	419887	7	NULL	NULL	NULL	NULL	 first word	Language												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In three experiments , participants were exposed to either alcohol or control beverage images , then asked to type as quickly as possible the first word that came to mind in response to a series of provocative ( e.g. , feces ) and neutral ( e.g. , chair ) stimulus words .
	manualset3
215843	6	419887	7	NULL	NULL	0	NULL	mind	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In three experiments , participants were exposed to either alcohol or control beverage images , then asked to type as quickly as possible the first word that came to mind in response to a series of provocative ( e.g. , feces ) and neutral ( e.g. , chair ) stimulus words .
	manualset3
215844	7	419887	7	NULL	NULL	0	NULL	series	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In three experiments , participants were exposed to either alcohol or control beverage images , then asked to type as quickly as possible the first word that came to mind in response to a series of provocative ( e.g. , feces ) and neutral ( e.g. , chair ) stimulus words .
	manualset3
215845	8	419887	7	NULL	NULL	NULL	NULL	provocative stimulus words	Language												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In three experiments , participants were exposed to either alcohol or control beverage images , then asked to type as quickly as possible the first word that came to mind in response to a series of provocative ( e.g. , feces ) and neutral ( e.g. , chair ) stimulus words .
	manualset3
215846	9	419887	7	NULL	NULL	0	NULL	feces	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In three experiments , participants were exposed to either alcohol or control beverage images , then asked to type as quickly as possible the first word that came to mind in response to a series of provocative ( e.g. , feces ) and neutral ( e.g. , chair ) stimulus words .
	manualset3
215847	10	419887	7	NULL	NULL	0	NULL	chair	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In three experiments , participants were exposed to either alcohol or control beverage images , then asked to type as quickly as possible the first word that came to mind in response to a series of provocative ( e.g. , feces ) and neutral ( e.g. , chair ) stimulus words .
	manualset3
215848	11	419887	7	NULL	NULL	NULL	NULL	neutral stimulus words	Language												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In three experiments , participants were exposed to either alcohol or control beverage images , then asked to type as quickly as possible the first word that came to mind in response to a series of provocative ( e.g. , feces ) and neutral ( e.g. , chair ) stimulus words .
	manualset3
215849	1	419888	7	NULL	NULL	0	NULL	condylar head	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the condylar head was returned to the glenoid fossa , optimal occlusion was not obtained because of compensatory tooth movement and inclination .
	manualset3
215850	2	419888	7	NULL	NULL	0	NULL	glenoid fossa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the condylar head was returned to the glenoid fossa , optimal occlusion was not obtained because of compensatory tooth movement and inclination .
	manualset3
215851	3	419888	7	NULL	NULL	0	NULL	optimal occlusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the condylar head was returned to the glenoid fossa , optimal occlusion was not obtained because of compensatory tooth movement and inclination .
	manualset3
215852	4	419888	7	NULL	NULL	0	NULL	compensatory tooth movement 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the condylar head was returned to the glenoid fossa , optimal occlusion was not obtained because of compensatory tooth movement and inclination .
	manualset3
215853	5	419888	7	NULL	NULL	0	NULL	 inclination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the condylar head was returned to the glenoid fossa , optimal occlusion was not obtained because of compensatory tooth movement and inclination .
	manualset3
215854	1	419889	7	NULL	NULL	0	NULL	Amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino acids , including taurine , that had not been determined previously in atrial gland vesicles were observed by using CE-LIF , and their identities were confirmed with CE , HPLC , NMR , and electrospray ionization mass spectrometry .
	manualset3
215855	2	419889	7	NULL	NULL	0	NULL	taurine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino acids , including taurine , that had not been determined previously in atrial gland vesicles were observed by using CE-LIF , and their identities were confirmed with CE , HPLC , NMR , and electrospray ionization mass spectrometry .
	manualset3
215856	3	419889	7	NULL	NULL	0	NULL	atrial gland vesicles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino acids , including taurine , that had not been determined previously in atrial gland vesicles were observed by using CE-LIF , and their identities were confirmed with CE , HPLC , NMR , and electrospray ionization mass spectrometry .
	manualset3
215857	4	419889	7	NULL	NULL	0	NULL	CE-LIF	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino acids , including taurine , that had not been determined previously in atrial gland vesicles were observed by using CE-LIF , and their identities were confirmed with CE , HPLC , NMR , and electrospray ionization mass spectrometry .
	manualset3
215858	5	419889	7	NULL	NULL	0	NULL	identities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino acids , including taurine , that had not been determined previously in atrial gland vesicles were observed by using CE-LIF , and their identities were confirmed with CE , HPLC , NMR , and electrospray ionization mass spectrometry .
	manualset3
215859	6	419889	7	NULL	NULL	0	NULL	CE	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino acids , including taurine , that had not been determined previously in atrial gland vesicles were observed by using CE-LIF , and their identities were confirmed with CE , HPLC , NMR , and electrospray ionization mass spectrometry .
	manualset3
215860	7	419889	7	NULL	NULL	0	NULL	HPLC	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino acids , including taurine , that had not been determined previously in atrial gland vesicles were observed by using CE-LIF , and their identities were confirmed with CE , HPLC , NMR , and electrospray ionization mass spectrometry .
	manualset3
215861	8	419889	7	NULL	NULL	0	NULL	NMR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino acids , including taurine , that had not been determined previously in atrial gland vesicles were observed by using CE-LIF , and their identities were confirmed with CE , HPLC , NMR , and electrospray ionization mass spectrometry .
	manualset3
215862	9	419889	7	NULL	NULL	0	NULL	 electrospray ionization mass spectrometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino acids , including taurine , that had not been determined previously in atrial gland vesicles were observed by using CE-LIF , and their identities were confirmed with CE , HPLC , NMR , and electrospray ionization mass spectrometry .
	manualset3
215863	1	419890	7	NULL	NULL	0	NULL	GDP-mannose mannosyl hydrolase ( GDPMH )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	GDP-mannose mannosyl hydrolase ( GDPMH ) is an unusual Nudix family member , which catalyzes the hydrolysis of GDP-alpha-D-mannose to GDP and the beta-sugar by nucleophilic substitution at carbon rather than at phosphorus ( Legler , P. M. , Massiah , M. A. , Bessman , M. J. , and Mildvan , A. S. ( 2000 ) Biochemistry 39 , 8603-8608 ) .
	manualset3
215864	2	419890	7	NULL	NULL	0	NULL	Nudix family member	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	GDP-mannose mannosyl hydrolase ( GDPMH ) is an unusual Nudix family member , which catalyzes the hydrolysis of GDP-alpha-D-mannose to GDP and the beta-sugar by nucleophilic substitution at carbon rather than at phosphorus ( Legler , P. M. , Massiah , M. A. , Bessman , M. J. , and Mildvan , A. S. ( 2000 ) Biochemistry 39 , 8603-8608 ) .
	manualset3
215865	3	419890	7	NULL	NULL	0	NULL	hydrolysis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GDP-mannose mannosyl hydrolase ( GDPMH ) is an unusual Nudix family member , which catalyzes the hydrolysis of GDP-alpha-D-mannose to GDP and the beta-sugar by nucleophilic substitution at carbon rather than at phosphorus ( Legler , P. M. , Massiah , M. A. , Bessman , M. J. , and Mildvan , A. S. ( 2000 ) Biochemistry 39 , 8603-8608 ) .
	manualset3
215866	4	419890	7	NULL	NULL	0	NULL	GDP-alpha-D-mannose	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	GDP-mannose mannosyl hydrolase ( GDPMH ) is an unusual Nudix family member , which catalyzes the hydrolysis of GDP-alpha-D-mannose to GDP and the beta-sugar by nucleophilic substitution at carbon rather than at phosphorus ( Legler , P. M. , Massiah , M. A. , Bessman , M. J. , and Mildvan , A. S. ( 2000 ) Biochemistry 39 , 8603-8608 ) .
	manualset3
215867	5	419890	7	NULL	NULL	0	NULL	GDP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	GDP-mannose mannosyl hydrolase ( GDPMH ) is an unusual Nudix family member , which catalyzes the hydrolysis of GDP-alpha-D-mannose to GDP and the beta-sugar by nucleophilic substitution at carbon rather than at phosphorus ( Legler , P. M. , Massiah , M. A. , Bessman , M. J. , and Mildvan , A. S. ( 2000 ) Biochemistry 39 , 8603-8608 ) .
	manualset3
215868	6	419890	7	NULL	NULL	0	NULL	beta-sugar	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	GDP-mannose mannosyl hydrolase ( GDPMH ) is an unusual Nudix family member , which catalyzes the hydrolysis of GDP-alpha-D-mannose to GDP and the beta-sugar by nucleophilic substitution at carbon rather than at phosphorus ( Legler , P. M. , Massiah , M. A. , Bessman , M. J. , and Mildvan , A. S. ( 2000 ) Biochemistry 39 , 8603-8608 ) .
	manualset3
215869	7	419890	7	NULL	NULL	0	NULL	nucleophilic substitution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	GDP-mannose mannosyl hydrolase ( GDPMH ) is an unusual Nudix family member , which catalyzes the hydrolysis of GDP-alpha-D-mannose to GDP and the beta-sugar by nucleophilic substitution at carbon rather than at phosphorus ( Legler , P. M. , Massiah , M. A. , Bessman , M. J. , and Mildvan , A. S. ( 2000 ) Biochemistry 39 , 8603-8608 ) .
	manualset3
215870	8	419890	7	NULL	NULL	0	NULL	carbon	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	GDP-mannose mannosyl hydrolase ( GDPMH ) is an unusual Nudix family member , which catalyzes the hydrolysis of GDP-alpha-D-mannose to GDP and the beta-sugar by nucleophilic substitution at carbon rather than at phosphorus ( Legler , P. M. , Massiah , M. A. , Bessman , M. J. , and Mildvan , A. S. ( 2000 ) Biochemistry 39 , 8603-8608 ) .
	manualset3
215871	9	419890	7	NULL	NULL	0	NULL	phosphorus	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	GDP-mannose mannosyl hydrolase ( GDPMH ) is an unusual Nudix family member , which catalyzes the hydrolysis of GDP-alpha-D-mannose to GDP and the beta-sugar by nucleophilic substitution at carbon rather than at phosphorus ( Legler , P. M. , Massiah , M. A. , Bessman , M. J. , and Mildvan , A. S. ( 2000 ) Biochemistry 39 , 8603-8608 ) .
	manualset3
215872	10	419890	7	NULL	NULL	0	NULL	Legler , P. M. , Massiah , M. A. , Bessman , M. J. , and Mildvan , A. S. ( 2000 ) Biochemistry 39 , 8603-8608	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	GDP-mannose mannosyl hydrolase ( GDPMH ) is an unusual Nudix family member , which catalyzes the hydrolysis of GDP-alpha-D-mannose to GDP and the beta-sugar by nucleophilic substitution at carbon rather than at phosphorus ( Legler , P. M. , Massiah , M. A. , Bessman , M. J. , and Mildvan , A. S. ( 2000 ) Biochemistry 39 , 8603-8608 ) .
	manualset3
215873	1	419891	7	NULL	NULL	0	NULL	open perspective	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In face of such an open perspective of basic and applied research , we review current evidence of lamin A/C interplay with signaling molecules , with particular emphasis on the lamin A-Akt interaction and on the biological significance of their relationship .
	manualset3
215874	2	419891	7	NULL	NULL	0	NULL	basic research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In face of such an open perspective of basic and applied research , we review current evidence of lamin A/C interplay with signaling molecules , with particular emphasis on the lamin A-Akt interaction and on the biological significance of their relationship .
	manualset3
215875	3	419891	7	NULL	NULL	0	NULL	applied research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In face of such an open perspective of basic and applied research , we review current evidence of lamin A/C interplay with signaling molecules , with particular emphasis on the lamin A-Akt interaction and on the biological significance of their relationship .
	manualset3
215876	4	419891	7	NULL	NULL	0	NULL	 current evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In face of such an open perspective of basic and applied research , we review current evidence of lamin A/C interplay with signaling molecules , with particular emphasis on the lamin A-Akt interaction and on the biological significance of their relationship .
	manualset3
215877	5	419891	7	NULL	NULL	0	NULL	lamin A/C interplay	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In face of such an open perspective of basic and applied research , we review current evidence of lamin A/C interplay with signaling molecules , with particular emphasis on the lamin A-Akt interaction and on the biological significance of their relationship .
	manualset3
215878	6	419891	7	NULL	NULL	0	NULL	signaling molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In face of such an open perspective of basic and applied research , we review current evidence of lamin A/C interplay with signaling molecules , with particular emphasis on the lamin A-Akt interaction and on the biological significance of their relationship .
	manualset3
215879	7	419891	7	NULL	NULL	0	NULL	 emphasis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In face of such an open perspective of basic and applied research , we review current evidence of lamin A/C interplay with signaling molecules , with particular emphasis on the lamin A-Akt interaction and on the biological significance of their relationship .
	manualset3
215880	8	419891	7	NULL	NULL	0	NULL	lamin A-Akt interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In face of such an open perspective of basic and applied research , we review current evidence of lamin A/C interplay with signaling molecules , with particular emphasis on the lamin A-Akt interaction and on the biological significance of their relationship .
	manualset3
215881	9	419891	7	NULL	NULL	0	NULL	 biological significance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In face of such an open perspective of basic and applied research , we review current evidence of lamin A/C interplay with signaling molecules , with particular emphasis on the lamin A-Akt interaction and on the biological significance of their relationship .
	manualset3
215882	10	419891	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In face of such an open perspective of basic and applied research , we review current evidence of lamin A/C interplay with signaling molecules , with particular emphasis on the lamin A-Akt interaction and on the biological significance of their relationship .
	manualset3
215883	1	419892	7	NULL	NULL	0	NULL	Subsistence ecology	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsistence ecology and carrying capacity in two Papua New Guinea populations .
	manualset3
215884	2	419892	7	NULL	NULL	0	NULL	carrying capacity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsistence ecology and carrying capacity in two Papua New Guinea populations .
	manualset3
215885	3	419892	7	NULL	NULL	0	NULL	two Papua New Guinea populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsistence ecology and carrying capacity in two Papua New Guinea populations .
	manualset3
215886	1	419893	7	NULL	NULL	0	NULL	Soft tissue opacification	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Soft tissue opacification did not alter the detectability of any nasal border structure lesion .
	manualset3
215887	2	419893	7	NULL	NULL	0	NULL	detectability 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Soft tissue opacification did not alter the detectability of any nasal border structure lesion .
	manualset3
215888	3	419893	7	NULL	NULL	0	NULL	nasal border structure lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Soft tissue opacification did not alter the detectability of any nasal border structure lesion .
	manualset3
215889	1	419894	7	NULL	NULL	0	NULL	His43	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	His43 is close to the C2 carbon of FPP and may stabilize the farnesyl cation intermediate during catalysis .
	manualset3
215890	2	419894	7	NULL	NULL	0	NULL	 C2 carbon	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	His43 is close to the C2 carbon of FPP and may stabilize the farnesyl cation intermediate during catalysis .
	manualset3
215891	3	419894	7	NULL	NULL	0	NULL	FPP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	His43 is close to the C2 carbon of FPP and may stabilize the farnesyl cation intermediate during catalysis .
	manualset3
215892	4	419894	7	NULL	NULL	0	NULL	farnesyl cation intermediate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	His43 is close to the C2 carbon of FPP and may stabilize the farnesyl cation intermediate during catalysis .
	manualset3
215893	5	419894	7	NULL	NULL	0	NULL	catalysis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	His43 is close to the C2 carbon of FPP and may stabilize the farnesyl cation intermediate during catalysis .
	manualset3
215894	1	419895	7	NULL	NULL	0	NULL	Serum CXCL10	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum CXCL10 was significantly associated with high pathological T stage , the presence of vascular invasion and distant metastasis .
	manualset3
215895	2	419895	7	NULL	NULL	0	NULL	high pathological T stage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum CXCL10 was significantly associated with high pathological T stage , the presence of vascular invasion and distant metastasis .
	manualset3
215896	3	419895	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum CXCL10 was significantly associated with high pathological T stage , the presence of vascular invasion and distant metastasis .
	manualset3
215897	4	419895	7	NULL	NULL	0	NULL	vascular invasion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum CXCL10 was significantly associated with high pathological T stage , the presence of vascular invasion and distant metastasis .
	manualset3
215898	5	419895	7	NULL	NULL	0	NULL	distant metastasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serum CXCL10 was significantly associated with high pathological T stage , the presence of vascular invasion and distant metastasis .
	manualset3
215899	1	419896	7	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the correlation between beta3-tubulin expression level in tumors has been well correlated with clinical outcome in patients receiving microtubule-targeted agents , the regulation of this protein remains poorly understood .
	manualset3
215900	2	419896	7	NULL	NULL	0	NULL	beta3-tubulin expression level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the correlation between beta3-tubulin expression level in tumors has been well correlated with clinical outcome in patients receiving microtubule-targeted agents , the regulation of this protein remains poorly understood .
	manualset3
215901	3	419896	7	NULL	NULL	0	NULL	 tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the correlation between beta3-tubulin expression level in tumors has been well correlated with clinical outcome in patients receiving microtubule-targeted agents , the regulation of this protein remains poorly understood .
	manualset3
215902	4	419896	7	NULL	NULL	0	NULL	clinical outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the correlation between beta3-tubulin expression level in tumors has been well correlated with clinical outcome in patients receiving microtubule-targeted agents , the regulation of this protein remains poorly understood .
	manualset3
215903	5	419896	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the correlation between beta3-tubulin expression level in tumors has been well correlated with clinical outcome in patients receiving microtubule-targeted agents , the regulation of this protein remains poorly understood .
	manualset3
215904	6	419896	7	NULL	NULL	0	NULL	microtubule-targeted agents	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the correlation between beta3-tubulin expression level in tumors has been well correlated with clinical outcome in patients receiving microtubule-targeted agents , the regulation of this protein remains poorly understood .
	manualset3
215905	7	419896	7	NULL	NULL	0	NULL	 regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the correlation between beta3-tubulin expression level in tumors has been well correlated with clinical outcome in patients receiving microtubule-targeted agents , the regulation of this protein remains poorly understood .
	manualset3
215906	8	419896	7	NULL	NULL	0	NULL	protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the correlation between beta3-tubulin expression level in tumors has been well correlated with clinical outcome in patients receiving microtubule-targeted agents , the regulation of this protein remains poorly understood .
	manualset3
215907	1	419897	7	NULL	NULL	0	NULL	 chemical synthesis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was prepared by chemical synthesis and tested for biological activity in in vitro lymphocyte culture systems .
	manualset3
215908	2	419897	7	NULL	NULL	0	NULL	biological activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was prepared by chemical synthesis and tested for biological activity in in vitro lymphocyte culture systems .
	manualset3
215909	3	419897	7	NULL	NULL	0	NULL	in vitro lymphocyte culture systems	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	It was prepared by chemical synthesis and tested for biological activity in in vitro lymphocyte culture systems .
	manualset3
215910	1	419898	7	NULL	NULL	0	NULL	Dipeptidyl peptidase-4 inhibitor 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Dipeptidyl peptidase-4 inhibitor another player for cardiovascular protection .
	manualset3
215911	2	419898	7	NULL	NULL	0	NULL	 player	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Dipeptidyl peptidase-4 inhibitor another player for cardiovascular protection .
	manualset3
215912	3	419898	7	NULL	NULL	0	NULL	 cardiovascular protection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dipeptidyl peptidase-4 inhibitor another player for cardiovascular protection .
	manualset3
215913	1	419899	7	NULL	NULL	0	NULL	relative frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative frequency with which patients who have these disorders develop PETs is MEN1 ) VHL ) NF-1 ) TSC .
	manualset3
215914	2	419899	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative frequency with which patients who have these disorders develop PETs is MEN1 ) VHL ) NF-1 ) TSC .
	manualset3
215915	3	419899	7	NULL	NULL	0	NULL	disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative frequency with which patients who have these disorders develop PETs is MEN1 ) VHL ) NF-1 ) TSC .
	manualset3
215916	4	419899	7	NULL	NULL	0	NULL	PETs	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative frequency with which patients who have these disorders develop PETs is MEN1 ) VHL ) NF-1 ) TSC .
	manualset3
215917	5	419899	7	NULL	NULL	0	NULL	MEN1	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative frequency with which patients who have these disorders develop PETs is MEN1 ) VHL ) NF-1 ) TSC .
	manualset3
215918	6	419899	7	NULL	NULL	0	NULL	 VHL	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative frequency with which patients who have these disorders develop PETs is MEN1 ) VHL ) NF-1 ) TSC .
	manualset3
215919	7	419899	7	NULL	NULL	0	NULL	NF-1	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative frequency with which patients who have these disorders develop PETs is MEN1 ) VHL ) NF-1 ) TSC .
	manualset3
215920	8	419899	7	NULL	NULL	0	NULL	TSC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative frequency with which patients who have these disorders develop PETs is MEN1 ) VHL ) NF-1 ) TSC .
	manualset3
215921	1	419900	7	NULL	NULL	0	NULL	phosphorylated Mcm2 ( pMcm2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We found phosphorylated Mcm2 ( pMcm2 ) markedly associated with neurofibrillary tangles , neuropil threads , and dystrophic neurites in AD but not in aged-matched controls .
	manualset3
215922	2	419900	7	NULL	NULL	0	NULL	neurofibrillary tangles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We found phosphorylated Mcm2 ( pMcm2 ) markedly associated with neurofibrillary tangles , neuropil threads , and dystrophic neurites in AD but not in aged-matched controls .
	manualset3
215923	3	419900	7	NULL	NULL	NULL	NULL	neuropil threads	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We found phosphorylated Mcm2 ( pMcm2 ) markedly associated with neurofibrillary tangles , neuropil threads , and dystrophic neurites in AD but not in aged-matched controls .
	manualset3
215924	4	419900	7	NULL	NULL	NULL	NULL	dystrophic neurites	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We found phosphorylated Mcm2 ( pMcm2 ) markedly associated with neurofibrillary tangles , neuropil threads , and dystrophic neurites in AD but not in aged-matched controls .
	manualset3
215925	5	419900	7	NULL	NULL	0	NULL	AD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We found phosphorylated Mcm2 ( pMcm2 ) markedly associated with neurofibrillary tangles , neuropil threads , and dystrophic neurites in AD but not in aged-matched controls .
	manualset3
215926	6	419900	7	NULL	NULL	0	NULL	aged-matched controls 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We found phosphorylated Mcm2 ( pMcm2 ) markedly associated with neurofibrillary tangles , neuropil threads , and dystrophic neurites in AD but not in aged-matched controls .
	manualset3
215927	1	419901	7	NULL	NULL	0	NULL	Z	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Z , in both a triacetylated and non-acetylated state , are used in native chromatin immmuno-precipitation experiments with mononucleosomes from three chicken cell types .
	manualset3
215928	2	419901	7	NULL	NULL	0	NULL	 triacetylated state	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Z , in both a triacetylated and non-acetylated state , are used in native chromatin immmuno-precipitation experiments with mononucleosomes from three chicken cell types .
	manualset3
215929	3	419901	7	NULL	NULL	0	NULL	non-acetylated state	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Z , in both a triacetylated and non-acetylated state , are used in native chromatin immmuno-precipitation experiments with mononucleosomes from three chicken cell types .
	manualset3
215930	4	419901	7	NULL	NULL	0	NULL	native chromatin immmuno-precipitation experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Z , in both a triacetylated and non-acetylated state , are used in native chromatin immmuno-precipitation experiments with mononucleosomes from three chicken cell types .
	manualset3
215931	5	419901	7	NULL	NULL	0	NULL	mononucleosomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Z , in both a triacetylated and non-acetylated state , are used in native chromatin immmuno-precipitation experiments with mononucleosomes from three chicken cell types .
	manualset3
215932	6	419901	7	NULL	NULL	0	NULL	three chicken cell types	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Z , in both a triacetylated and non-acetylated state , are used in native chromatin immmuno-precipitation experiments with mononucleosomes from three chicken cell types .
	manualset3
215933	1	419902	7	NULL	NULL	0	NULL	Biochemical markers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Biochemical markers of inflammation are emerging as new predictors of risk of cardiovascular disease ( CVD ) and may alter acutely with exercise .
	manualset3
215934	2	419902	7	NULL	NULL	0	NULL	inflammation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Biochemical markers of inflammation are emerging as new predictors of risk of cardiovascular disease ( CVD ) and may alter acutely with exercise .
	manualset3
215935	3	419902	7	NULL	NULL	0	NULL	new predictors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Biochemical markers of inflammation are emerging as new predictors of risk of cardiovascular disease ( CVD ) and may alter acutely with exercise .
	manualset3
215936	4	419902	7	NULL	NULL	0	NULL	risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Biochemical markers of inflammation are emerging as new predictors of risk of cardiovascular disease ( CVD ) and may alter acutely with exercise .
	manualset3
215937	5	419902	7	NULL	NULL	0	NULL	cardiovascular disease ( CVD ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Biochemical markers of inflammation are emerging as new predictors of risk of cardiovascular disease ( CVD ) and may alter acutely with exercise .
	manualset3
215938	6	419902	7	NULL	NULL	0	NULL	exercise	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Biochemical markers of inflammation are emerging as new predictors of risk of cardiovascular disease ( CVD ) and may alter acutely with exercise .
	manualset3
215939	1	419903	7	NULL	NULL	0	NULL	attempt	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An attempt was made to calculate the change of the partial specific volume of hemocyanin by adding glycerol or saccharose .
	manualset3
215940	2	419903	7	NULL	NULL	0	NULL	change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An attempt was made to calculate the change of the partial specific volume of hemocyanin by adding glycerol or saccharose .
	manualset3
215941	3	419903	7	NULL	NULL	0	NULL	partial specific volume	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An attempt was made to calculate the change of the partial specific volume of hemocyanin by adding glycerol or saccharose .
	manualset3
215942	4	419903	7	NULL	NULL	0	NULL	hemocyanin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An attempt was made to calculate the change of the partial specific volume of hemocyanin by adding glycerol or saccharose .
	manualset3
215943	5	419903	7	NULL	NULL	0	NULL	glycerol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An attempt was made to calculate the change of the partial specific volume of hemocyanin by adding glycerol or saccharose .
	manualset3
215944	6	419903	7	NULL	NULL	0	NULL	saccharose 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An attempt was made to calculate the change of the partial specific volume of hemocyanin by adding glycerol or saccharose .
	manualset3
215945	1	419904	7	NULL	NULL	0	NULL	Deconjugation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Deconjugation of hydroquinone likely is catalyzed by intracellular enzymes presumably present in bacterial cytoplasm ; comparable activities in eucaryotic cells usually are localized in lysosomes .
	manualset3
215946	2	419904	7	NULL	NULL	0	NULL	 hydroquinone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Deconjugation of hydroquinone likely is catalyzed by intracellular enzymes presumably present in bacterial cytoplasm ; comparable activities in eucaryotic cells usually are localized in lysosomes .
	manualset3
215947	3	419904	7	NULL	NULL	0	NULL	intracellular enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Deconjugation of hydroquinone likely is catalyzed by intracellular enzymes presumably present in bacterial cytoplasm ; comparable activities in eucaryotic cells usually are localized in lysosomes .
	manualset3
215948	4	419904	7	NULL	NULL	0	NULL	bacterial cytoplasm	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Deconjugation of hydroquinone likely is catalyzed by intracellular enzymes presumably present in bacterial cytoplasm ; comparable activities in eucaryotic cells usually are localized in lysosomes .
	manualset3
215949	5	419904	7	NULL	NULL	0	NULL	comparable activities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Deconjugation of hydroquinone likely is catalyzed by intracellular enzymes presumably present in bacterial cytoplasm ; comparable activities in eucaryotic cells usually are localized in lysosomes .
	manualset3
215950	6	419904	7	NULL	NULL	0	NULL	eucaryotic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Deconjugation of hydroquinone likely is catalyzed by intracellular enzymes presumably present in bacterial cytoplasm ; comparable activities in eucaryotic cells usually are localized in lysosomes .
	manualset3
215951	7	419904	7	NULL	NULL	0	NULL	lysosomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Deconjugation of hydroquinone likely is catalyzed by intracellular enzymes presumably present in bacterial cytoplasm ; comparable activities in eucaryotic cells usually are localized in lysosomes .
	manualset3
215952	1	419905	7	NULL	NULL	0	NULL	defining feature 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the defining feature of these approaches is the systematic identification of environmental determinants of behavior , research methodology has varied widely with respect to the arrangements used to demonstrate experimental control as well as the types of variables subject to analysis .
	manualset3
215953	2	419905	7	NULL	NULL	0	NULL	 approaches	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the defining feature of these approaches is the systematic identification of environmental determinants of behavior , research methodology has varied widely with respect to the arrangements used to demonstrate experimental control as well as the types of variables subject to analysis .
	manualset3
215954	3	419905	7	NULL	NULL	0	NULL	systematic identification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the defining feature of these approaches is the systematic identification of environmental determinants of behavior , research methodology has varied widely with respect to the arrangements used to demonstrate experimental control as well as the types of variables subject to analysis .
	manualset3
215955	4	419905	7	NULL	NULL	0	NULL	environmental determinants	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the defining feature of these approaches is the systematic identification of environmental determinants of behavior , research methodology has varied widely with respect to the arrangements used to demonstrate experimental control as well as the types of variables subject to analysis .
	manualset3
215956	5	419905	7	NULL	NULL	0	NULL	behavior	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the defining feature of these approaches is the systematic identification of environmental determinants of behavior , research methodology has varied widely with respect to the arrangements used to demonstrate experimental control as well as the types of variables subject to analysis .
	manualset3
215957	6	419905	7	NULL	NULL	0	NULL	research methodology	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the defining feature of these approaches is the systematic identification of environmental determinants of behavior , research methodology has varied widely with respect to the arrangements used to demonstrate experimental control as well as the types of variables subject to analysis .
	manualset3
215958	7	419905	7	NULL	NULL	0	NULL	arrangements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the defining feature of these approaches is the systematic identification of environmental determinants of behavior , research methodology has varied widely with respect to the arrangements used to demonstrate experimental control as well as the types of variables subject to analysis .
	manualset3
215959	8	419905	7	NULL	NULL	0	NULL	experimental control 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the defining feature of these approaches is the systematic identification of environmental determinants of behavior , research methodology has varied widely with respect to the arrangements used to demonstrate experimental control as well as the types of variables subject to analysis .
	manualset3
215960	9	419905	7	NULL	NULL	0	NULL	types of variables	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the defining feature of these approaches is the systematic identification of environmental determinants of behavior , research methodology has varied widely with respect to the arrangements used to demonstrate experimental control as well as the types of variables subject to analysis .
	manualset3
215961	10	419905	7	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the defining feature of these approaches is the systematic identification of environmental determinants of behavior , research methodology has varied widely with respect to the arrangements used to demonstrate experimental control as well as the types of variables subject to analysis .
	manualset3
215962	1	419906	7	NULL	NULL	0	NULL	 kinetics	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We find that these kinetics were slightly less sensitive to temperature than was the unloaded shortening speed .
	manualset3
215963	2	419906	7	NULL	NULL	0	NULL	 temperature	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We find that these kinetics were slightly less sensitive to temperature than was the unloaded shortening speed .
	manualset3
215964	3	419906	7	NULL	NULL	0	NULL	unloaded shortening speed	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We find that these kinetics were slightly less sensitive to temperature than was the unloaded shortening speed .
	manualset3
215965	1	419907	7	NULL	NULL	0	NULL	Results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results for this sample of children indicated that the PLL was similar to the DSL targets , and that , on average , NAL-RP/NL1 targets recommended less gain than that preferred by the majority of children in this study .
	manualset3
215966	2	419907	7	NULL	NULL	0	NULL	sample of children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results for this sample of children indicated that the PLL was similar to the DSL targets , and that , on average , NAL-RP/NL1 targets recommended less gain than that preferred by the majority of children in this study .
	manualset3
215967	3	419907	7	NULL	NULL	0	NULL	PLL	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results for this sample of children indicated that the PLL was similar to the DSL targets , and that , on average , NAL-RP/NL1 targets recommended less gain than that preferred by the majority of children in this study .
	manualset3
215968	4	419907	7	NULL	NULL	0	NULL	 DSL targets	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results for this sample of children indicated that the PLL was similar to the DSL targets , and that , on average , NAL-RP/NL1 targets recommended less gain than that preferred by the majority of children in this study .
	manualset3
215969	5	419907	7	NULL	NULL	0	NULL	NAL-RP/NL1 targets	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results for this sample of children indicated that the PLL was similar to the DSL targets , and that , on average , NAL-RP/NL1 targets recommended less gain than that preferred by the majority of children in this study .
	manualset3
215970	6	419907	7	NULL	NULL	0	NULL	majority	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results for this sample of children indicated that the PLL was similar to the DSL targets , and that , on average , NAL-RP/NL1 targets recommended less gain than that preferred by the majority of children in this study .
	manualset3
215971	7	419907	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results for this sample of children indicated that the PLL was similar to the DSL targets , and that , on average , NAL-RP/NL1 targets recommended less gain than that preferred by the majority of children in this study .
	manualset3
215972	8	419907	7	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results for this sample of children indicated that the PLL was similar to the DSL targets , and that , on average , NAL-RP/NL1 targets recommended less gain than that preferred by the majority of children in this study .
	manualset3
215973	1	419908	7	NULL	NULL	0	NULL	 role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To further define the role of chemokines in leukocyte recruitment into tumors , we evaluated anti-tumor responses in mice lacking the chemokine receptor , CCR2 .
	manualset3
215974	2	419908	7	NULL	NULL	0	NULL	chemokines 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To further define the role of chemokines in leukocyte recruitment into tumors , we evaluated anti-tumor responses in mice lacking the chemokine receptor , CCR2 .
	manualset3
215975	3	419908	7	NULL	NULL	0	NULL	leukocyte recruitment	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To further define the role of chemokines in leukocyte recruitment into tumors , we evaluated anti-tumor responses in mice lacking the chemokine receptor , CCR2 .
	manualset3
215976	4	419908	7	NULL	NULL	0	NULL	tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To further define the role of chemokines in leukocyte recruitment into tumors , we evaluated anti-tumor responses in mice lacking the chemokine receptor , CCR2 .
	manualset3
215977	5	419908	7	NULL	NULL	0	NULL	anti-tumor responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To further define the role of chemokines in leukocyte recruitment into tumors , we evaluated anti-tumor responses in mice lacking the chemokine receptor , CCR2 .
	manualset3
215978	6	419908	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To further define the role of chemokines in leukocyte recruitment into tumors , we evaluated anti-tumor responses in mice lacking the chemokine receptor , CCR2 .
	manualset3
215979	7	419908	7	NULL	NULL	0	NULL	chemokine receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To further define the role of chemokines in leukocyte recruitment into tumors , we evaluated anti-tumor responses in mice lacking the chemokine receptor , CCR2 .
	manualset3
215980	8	419908	7	NULL	NULL	0	NULL	CCR2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To further define the role of chemokines in leukocyte recruitment into tumors , we evaluated anti-tumor responses in mice lacking the chemokine receptor , CCR2 .
	manualset3
215981	1	419909	7	NULL	NULL	0	NULL	tendency	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The tendency for rural South Indian women to prefer smaller babies and the relationship of this preference to dietary behavior are considered in relation to both concepts of the appropriate quality and quantity of food to eat during pregnancy and the concepts of baby space and baby strength .
	manualset3
215982	2	419909	7	NULL	NULL	0	NULL	rural South Indian women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The tendency for rural South Indian women to prefer smaller babies and the relationship of this preference to dietary behavior are considered in relation to both concepts of the appropriate quality and quantity of food to eat during pregnancy and the concepts of baby space and baby strength .
	manualset3
215983	3	419909	7	NULL	NULL	0	NULL	smaller babies	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The tendency for rural South Indian women to prefer smaller babies and the relationship of this preference to dietary behavior are considered in relation to both concepts of the appropriate quality and quantity of food to eat during pregnancy and the concepts of baby space and baby strength .
	manualset3
215984	4	419909	7	NULL	NULL	0	NULL	 relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The tendency for rural South Indian women to prefer smaller babies and the relationship of this preference to dietary behavior are considered in relation to both concepts of the appropriate quality and quantity of food to eat during pregnancy and the concepts of baby space and baby strength .
	manualset3
215985	5	419909	7	NULL	NULL	0	NULL	preference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The tendency for rural South Indian women to prefer smaller babies and the relationship of this preference to dietary behavior are considered in relation to both concepts of the appropriate quality and quantity of food to eat during pregnancy and the concepts of baby space and baby strength .
	manualset3
215986	6	419909	7	NULL	NULL	0	NULL	dietary behavior	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The tendency for rural South Indian women to prefer smaller babies and the relationship of this preference to dietary behavior are considered in relation to both concepts of the appropriate quality and quantity of food to eat during pregnancy and the concepts of baby space and baby strength .
	manualset3
215987	7	419909	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The tendency for rural South Indian women to prefer smaller babies and the relationship of this preference to dietary behavior are considered in relation to both concepts of the appropriate quality and quantity of food to eat during pregnancy and the concepts of baby space and baby strength .
	manualset3
215988	8	419909	7	NULL	NULL	0	NULL	concepts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The tendency for rural South Indian women to prefer smaller babies and the relationship of this preference to dietary behavior are considered in relation to both concepts of the appropriate quality and quantity of food to eat during pregnancy and the concepts of baby space and baby strength .
	manualset3
215989	9	419909	7	NULL	NULL	0	NULL	quality	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The tendency for rural South Indian women to prefer smaller babies and the relationship of this preference to dietary behavior are considered in relation to both concepts of the appropriate quality and quantity of food to eat during pregnancy and the concepts of baby space and baby strength .
	manualset3
215990	10	419909	7	NULL	NULL	0	NULL	 quantity 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The tendency for rural South Indian women to prefer smaller babies and the relationship of this preference to dietary behavior are considered in relation to both concepts of the appropriate quality and quantity of food to eat during pregnancy and the concepts of baby space and baby strength .
	manualset3
215991	11	419909	7	NULL	NULL	0	NULL	food	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The tendency for rural South Indian women to prefer smaller babies and the relationship of this preference to dietary behavior are considered in relation to both concepts of the appropriate quality and quantity of food to eat during pregnancy and the concepts of baby space and baby strength .
	manualset3
215992	12	419909	7	NULL	NULL	0	NULL	pregnancy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The tendency for rural South Indian women to prefer smaller babies and the relationship of this preference to dietary behavior are considered in relation to both concepts of the appropriate quality and quantity of food to eat during pregnancy and the concepts of baby space and baby strength .
	manualset3
215993	13	419909	7	NULL	NULL	0	NULL	concepts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The tendency for rural South Indian women to prefer smaller babies and the relationship of this preference to dietary behavior are considered in relation to both concepts of the appropriate quality and quantity of food to eat during pregnancy and the concepts of baby space and baby strength .
	manualset3
215994	14	419909	7	NULL	NULL	0	NULL	baby space	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The tendency for rural South Indian women to prefer smaller babies and the relationship of this preference to dietary behavior are considered in relation to both concepts of the appropriate quality and quantity of food to eat during pregnancy and the concepts of baby space and baby strength .
	manualset3
215995	15	419909	7	NULL	NULL	0	NULL	baby strength	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The tendency for rural South Indian women to prefer smaller babies and the relationship of this preference to dietary behavior are considered in relation to both concepts of the appropriate quality and quantity of food to eat during pregnancy and the concepts of baby space and baby strength .
	manualset3
215996	1	419910	7	NULL	NULL	0	NULL	lactation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	During lactation , all H sows were fed ad libitum ( H-AL ) whereas M sows were fed either ad libitum ( M-AL , n = 8 ) or were restricted ( M-RE , n = 8 ) to the amount of feed ingested by H-AL sows .
	manualset3
215997	2	419910	7	NULL	NULL	0	NULL	H sows 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	During lactation , all H sows were fed ad libitum ( H-AL ) whereas M sows were fed either ad libitum ( M-AL , n = 8 ) or were restricted ( M-RE , n = 8 ) to the amount of feed ingested by H-AL sows .
	manualset3
215998	3	419910	7	NULL	NULL	NULL	NULL	ad libitum ( H-AL )	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During lactation , all H sows were fed ad libitum ( H-AL ) whereas M sows were fed either ad libitum ( M-AL , n = 8 ) or were restricted ( M-RE , n = 8 ) to the amount of feed ingested by H-AL sows .
	manualset3
215999	4	419910	7	NULL	NULL	0	NULL	M sows	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	During lactation , all H sows were fed ad libitum ( H-AL ) whereas M sows were fed either ad libitum ( M-AL , n = 8 ) or were restricted ( M-RE , n = 8 ) to the amount of feed ingested by H-AL sows .
	manualset3
216000	5	419910	7	NULL	NULL	NULL	NULL	ad libitum	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During lactation , all H sows were fed ad libitum ( H-AL ) whereas M sows were fed either ad libitum ( M-AL , n = 8 ) or were restricted ( M-RE , n = 8 ) to the amount of feed ingested by H-AL sows .
	manualset3
216001	6	419910	7	NULL	NULL	0	NULL	M-AL	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	During lactation , all H sows were fed ad libitum ( H-AL ) whereas M sows were fed either ad libitum ( M-AL , n = 8 ) or were restricted ( M-RE , n = 8 ) to the amount of feed ingested by H-AL sows .
	manualset3
216002	7	419910	7	NULL	NULL	0	NULL	n = 8	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During lactation , all H sows were fed ad libitum ( H-AL ) whereas M sows were fed either ad libitum ( M-AL , n = 8 ) or were restricted ( M-RE , n = 8 ) to the amount of feed ingested by H-AL sows .
	manualset3
216003	8	419910	7	NULL	NULL	0	NULL	 M-RE	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	During lactation , all H sows were fed ad libitum ( H-AL ) whereas M sows were fed either ad libitum ( M-AL , n = 8 ) or were restricted ( M-RE , n = 8 ) to the amount of feed ingested by H-AL sows .
	manualset3
216004	9	419910	7	NULL	NULL	0	NULL	n = 8	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During lactation , all H sows were fed ad libitum ( H-AL ) whereas M sows were fed either ad libitum ( M-AL , n = 8 ) or were restricted ( M-RE , n = 8 ) to the amount of feed ingested by H-AL sows .
	manualset3
216005	10	419910	7	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	During lactation , all H sows were fed ad libitum ( H-AL ) whereas M sows were fed either ad libitum ( M-AL , n = 8 ) or were restricted ( M-RE , n = 8 ) to the amount of feed ingested by H-AL sows .
	manualset3
216006	11	419910	7	NULL	NULL	0	NULL	feed 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	During lactation , all H sows were fed ad libitum ( H-AL ) whereas M sows were fed either ad libitum ( M-AL , n = 8 ) or were restricted ( M-RE , n = 8 ) to the amount of feed ingested by H-AL sows .
	manualset3
216007	12	419910	7	NULL	NULL	0	NULL	H-AL sows	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	During lactation , all H sows were fed ad libitum ( H-AL ) whereas M sows were fed either ad libitum ( M-AL , n = 8 ) or were restricted ( M-RE , n = 8 ) to the amount of feed ingested by H-AL sows .
	manualset3
216008	1	419911	7	NULL	NULL	0	NULL	degree	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the degree of charge transfer between the rings is very small , as revealed by a Mulliken-Hash analysis , the split Cotton effects are due to a large separation in energy of the donor and acceptor orbitals .
	manualset3
216009	2	419911	7	NULL	NULL	0	NULL	charge transfer	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the degree of charge transfer between the rings is very small , as revealed by a Mulliken-Hash analysis , the split Cotton effects are due to a large separation in energy of the donor and acceptor orbitals .
	manualset3
216010	3	419911	7	NULL	NULL	0	NULL	rings	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the degree of charge transfer between the rings is very small , as revealed by a Mulliken-Hash analysis , the split Cotton effects are due to a large separation in energy of the donor and acceptor orbitals .
	manualset3
216011	4	419911	7	NULL	NULL	0	NULL	small	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the degree of charge transfer between the rings is very small , as revealed by a Mulliken-Hash analysis , the split Cotton effects are due to a large separation in energy of the donor and acceptor orbitals .
	manualset3
216012	5	419911	7	NULL	NULL	0	NULL	Mulliken-Hash analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the degree of charge transfer between the rings is very small , as revealed by a Mulliken-Hash analysis , the split Cotton effects are due to a large separation in energy of the donor and acceptor orbitals .
	manualset3
216013	6	419911	7	NULL	NULL	0	NULL	split Cotton effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the degree of charge transfer between the rings is very small , as revealed by a Mulliken-Hash analysis , the split Cotton effects are due to a large separation in energy of the donor and acceptor orbitals .
	manualset3
216014	7	419911	7	NULL	NULL	0	NULL	large separation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the degree of charge transfer between the rings is very small , as revealed by a Mulliken-Hash analysis , the split Cotton effects are due to a large separation in energy of the donor and acceptor orbitals .
	manualset3
216015	8	419911	7	NULL	NULL	0	NULL	energy	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the degree of charge transfer between the rings is very small , as revealed by a Mulliken-Hash analysis , the split Cotton effects are due to a large separation in energy of the donor and acceptor orbitals .
	manualset3
216016	9	419911	7	NULL	NULL	0	NULL	donor orbitals	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the degree of charge transfer between the rings is very small , as revealed by a Mulliken-Hash analysis , the split Cotton effects are due to a large separation in energy of the donor and acceptor orbitals .
	manualset3
216017	10	419911	7	NULL	NULL	0	NULL	acceptor orbitals	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the degree of charge transfer between the rings is very small , as revealed by a Mulliken-Hash analysis , the split Cotton effects are due to a large separation in energy of the donor and acceptor orbitals .
	manualset3
216018	1	419912	7	NULL	NULL	0	NULL	 data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the present data suggest a potential for anti-hIL-6 therapy in B-cell lymphomas .
	manualset3
216019	2	419912	7	NULL	NULL	0	NULL	 potential	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the present data suggest a potential for anti-hIL-6 therapy in B-cell lymphomas .
	manualset3
216020	3	419912	7	NULL	NULL	0	NULL	anti-hIL-6 therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the present data suggest a potential for anti-hIL-6 therapy in B-cell lymphomas .
	manualset3
216021	4	419912	7	NULL	NULL	0	NULL	B-cell lymphomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the present data suggest a potential for anti-hIL-6 therapy in B-cell lymphomas .
	manualset3
216022	1	419913	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to eight mismatches , mouse-virulent strains harbored five copies of an up-stream 27-bp repeat in the promotor region of SAG1 as compared with four copies in avirulent strains .
	manualset3
216023	2	419913	7	NULL	NULL	0	NULL	eight mismatches	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to eight mismatches , mouse-virulent strains harbored five copies of an up-stream 27-bp repeat in the promotor region of SAG1 as compared with four copies in avirulent strains .
	manualset3
216024	3	419913	7	NULL	NULL	0	NULL	mouse-virulent strains 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to eight mismatches , mouse-virulent strains harbored five copies of an up-stream 27-bp repeat in the promotor region of SAG1 as compared with four copies in avirulent strains .
	manualset3
216025	4	419913	7	NULL	NULL	0	NULL	five copies	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to eight mismatches , mouse-virulent strains harbored five copies of an up-stream 27-bp repeat in the promotor region of SAG1 as compared with four copies in avirulent strains .
	manualset3
216026	5	419913	7	NULL	NULL	0	NULL	up-stream 27-bp repeat	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to eight mismatches , mouse-virulent strains harbored five copies of an up-stream 27-bp repeat in the promotor region of SAG1 as compared with four copies in avirulent strains .
	manualset3
216027	6	419913	7	NULL	NULL	0	NULL	 promotor region 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to eight mismatches , mouse-virulent strains harbored five copies of an up-stream 27-bp repeat in the promotor region of SAG1 as compared with four copies in avirulent strains .
	manualset3
216028	7	419913	7	NULL	NULL	0	NULL	 SAG1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to eight mismatches , mouse-virulent strains harbored five copies of an up-stream 27-bp repeat in the promotor region of SAG1 as compared with four copies in avirulent strains .
	manualset3
216029	8	419913	7	NULL	NULL	0	NULL	four copies	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to eight mismatches , mouse-virulent strains harbored five copies of an up-stream 27-bp repeat in the promotor region of SAG1 as compared with four copies in avirulent strains .
	manualset3
216030	9	419913	7	NULL	NULL	0	NULL	avirulent strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to eight mismatches , mouse-virulent strains harbored five copies of an up-stream 27-bp repeat in the promotor region of SAG1 as compared with four copies in avirulent strains .
	manualset3
216031	1	419914	7	NULL	NULL	0	NULL	occurrence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The occurrence of interstitial lung disease similar to hard metal lung disease in diamond polishers who had been exposed to cobalt ( in the absence of tungsten carbide ) through the use of polishing disks containing microdiamonds sintered with cobalt , led us to experimentally test the hypothesis that cobalt has pro-oxidant activity in lung tissue .
	manualset3
216032	2	419914	7	NULL	NULL	0	NULL	interstitial lung disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The occurrence of interstitial lung disease similar to hard metal lung disease in diamond polishers who had been exposed to cobalt ( in the absence of tungsten carbide ) through the use of polishing disks containing microdiamonds sintered with cobalt , led us to experimentally test the hypothesis that cobalt has pro-oxidant activity in lung tissue .
	manualset3
216033	3	419914	7	NULL	NULL	0	NULL	hard metal lung disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The occurrence of interstitial lung disease similar to hard metal lung disease in diamond polishers who had been exposed to cobalt ( in the absence of tungsten carbide ) through the use of polishing disks containing microdiamonds sintered with cobalt , led us to experimentally test the hypothesis that cobalt has pro-oxidant activity in lung tissue .
	manualset3
216034	4	419914	7	NULL	NULL	0	NULL	diamond polishers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The occurrence of interstitial lung disease similar to hard metal lung disease in diamond polishers who had been exposed to cobalt ( in the absence of tungsten carbide ) through the use of polishing disks containing microdiamonds sintered with cobalt , led us to experimentally test the hypothesis that cobalt has pro-oxidant activity in lung tissue .
	manualset3
216035	5	419914	7	NULL	NULL	0	NULL	cobalt	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The occurrence of interstitial lung disease similar to hard metal lung disease in diamond polishers who had been exposed to cobalt ( in the absence of tungsten carbide ) through the use of polishing disks containing microdiamonds sintered with cobalt , led us to experimentally test the hypothesis that cobalt has pro-oxidant activity in lung tissue .
	manualset3
216036	6	419914	7	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The occurrence of interstitial lung disease similar to hard metal lung disease in diamond polishers who had been exposed to cobalt ( in the absence of tungsten carbide ) through the use of polishing disks containing microdiamonds sintered with cobalt , led us to experimentally test the hypothesis that cobalt has pro-oxidant activity in lung tissue .
	manualset3
216037	7	419914	7	NULL	NULL	0	NULL	tungsten carbide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The occurrence of interstitial lung disease similar to hard metal lung disease in diamond polishers who had been exposed to cobalt ( in the absence of tungsten carbide ) through the use of polishing disks containing microdiamonds sintered with cobalt , led us to experimentally test the hypothesis that cobalt has pro-oxidant activity in lung tissue .
	manualset3
216038	8	419914	7	NULL	NULL	0	NULL	use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The occurrence of interstitial lung disease similar to hard metal lung disease in diamond polishers who had been exposed to cobalt ( in the absence of tungsten carbide ) through the use of polishing disks containing microdiamonds sintered with cobalt , led us to experimentally test the hypothesis that cobalt has pro-oxidant activity in lung tissue .
	manualset3
216039	9	419914	7	NULL	NULL	0	NULL	polishing disks	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The occurrence of interstitial lung disease similar to hard metal lung disease in diamond polishers who had been exposed to cobalt ( in the absence of tungsten carbide ) through the use of polishing disks containing microdiamonds sintered with cobalt , led us to experimentally test the hypothesis that cobalt has pro-oxidant activity in lung tissue .
	manualset3
216040	10	419914	7	NULL	NULL	0	NULL	microdiamonds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The occurrence of interstitial lung disease similar to hard metal lung disease in diamond polishers who had been exposed to cobalt ( in the absence of tungsten carbide ) through the use of polishing disks containing microdiamonds sintered with cobalt , led us to experimentally test the hypothesis that cobalt has pro-oxidant activity in lung tissue .
	manualset3
216041	11	419914	7	NULL	NULL	0	NULL	cobalt	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The occurrence of interstitial lung disease similar to hard metal lung disease in diamond polishers who had been exposed to cobalt ( in the absence of tungsten carbide ) through the use of polishing disks containing microdiamonds sintered with cobalt , led us to experimentally test the hypothesis that cobalt has pro-oxidant activity in lung tissue .
	manualset3
216042	12	419914	7	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The occurrence of interstitial lung disease similar to hard metal lung disease in diamond polishers who had been exposed to cobalt ( in the absence of tungsten carbide ) through the use of polishing disks containing microdiamonds sintered with cobalt , led us to experimentally test the hypothesis that cobalt has pro-oxidant activity in lung tissue .
	manualset3
216043	13	419914	7	NULL	NULL	0	NULL	cobalt 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The occurrence of interstitial lung disease similar to hard metal lung disease in diamond polishers who had been exposed to cobalt ( in the absence of tungsten carbide ) through the use of polishing disks containing microdiamonds sintered with cobalt , led us to experimentally test the hypothesis that cobalt has pro-oxidant activity in lung tissue .
	manualset3
216044	14	419914	7	NULL	NULL	0	NULL	pro-oxidant activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The occurrence of interstitial lung disease similar to hard metal lung disease in diamond polishers who had been exposed to cobalt ( in the absence of tungsten carbide ) through the use of polishing disks containing microdiamonds sintered with cobalt , led us to experimentally test the hypothesis that cobalt has pro-oxidant activity in lung tissue .
	manualset3
216045	15	419914	7	NULL	NULL	0	NULL	lung tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The occurrence of interstitial lung disease similar to hard metal lung disease in diamond polishers who had been exposed to cobalt ( in the absence of tungsten carbide ) through the use of polishing disks containing microdiamonds sintered with cobalt , led us to experimentally test the hypothesis that cobalt has pro-oxidant activity in lung tissue .
	manualset3
216046	1	419915	7	NULL	NULL	0	NULL	Updated meta analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Updated meta analysis finds that interferon-alpha improves progression-free and overall survival in low-grade non-Hodgkin 's lymphoma when administered with chemotherapy that contains anthracycline or mitoxantrone .
	manualset3
216047	2	419915	7	NULL	NULL	0	NULL	 interferon-alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Updated meta analysis finds that interferon-alpha improves progression-free and overall survival in low-grade non-Hodgkin 's lymphoma when administered with chemotherapy that contains anthracycline or mitoxantrone .
	manualset3
216048	3	419915	7	NULL	NULL	0	NULL	progression-free survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Updated meta analysis finds that interferon-alpha improves progression-free and overall survival in low-grade non-Hodgkin 's lymphoma when administered with chemotherapy that contains anthracycline or mitoxantrone .
	manualset3
216049	4	419915	7	NULL	NULL	0	NULL	overall survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Updated meta analysis finds that interferon-alpha improves progression-free and overall survival in low-grade non-Hodgkin 's lymphoma when administered with chemotherapy that contains anthracycline or mitoxantrone .
	manualset3
216050	5	419915	7	NULL	NULL	0	NULL	low-grade non-Hodgkin 's lymphoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Updated meta analysis finds that interferon-alpha improves progression-free and overall survival in low-grade non-Hodgkin 's lymphoma when administered with chemotherapy that contains anthracycline or mitoxantrone .
	manualset3
216051	6	419915	7	NULL	NULL	0	NULL	chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Updated meta analysis finds that interferon-alpha improves progression-free and overall survival in low-grade non-Hodgkin 's lymphoma when administered with chemotherapy that contains anthracycline or mitoxantrone .
	manualset3
216052	7	419915	7	NULL	NULL	0	NULL	anthracycline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Updated meta analysis finds that interferon-alpha improves progression-free and overall survival in low-grade non-Hodgkin 's lymphoma when administered with chemotherapy that contains anthracycline or mitoxantrone .
	manualset3
216053	8	419915	7	NULL	NULL	0	NULL	 mitoxantrone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Updated meta analysis finds that interferon-alpha improves progression-free and overall survival in low-grade non-Hodgkin 's lymphoma when administered with chemotherapy that contains anthracycline or mitoxantrone .
	manualset3
216054	1	419916	7	NULL	NULL	0	NULL	K2P distances	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	K2P distances were calculated and NJ tree was performed by MEGA 4.1 .
	manualset3
216055	2	419916	7	NULL	NULL	0	NULL	NJ tree	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	K2P distances were calculated and NJ tree was performed by MEGA 4.1 .
	manualset3
216056	3	419916	7	NULL	NULL	0	NULL	MEGA 4.1	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	K2P distances were calculated and NJ tree was performed by MEGA 4.1 .
	manualset3
216057	1	419917	7	NULL	NULL	0	NULL	phenanthrene biodegradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The phenanthrene biodegradation could be best described by the first order rate model , C = C ( 0 ) e ( - kt ) , where k ( the rate constant ) is equaled to 0.1185 , under the optimal condition .
	manualset3
216058	2	419917	7	NULL	NULL	0	NULL	first order rate model 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The phenanthrene biodegradation could be best described by the first order rate model , C = C ( 0 ) e ( - kt ) , where k ( the rate constant ) is equaled to 0.1185 , under the optimal condition .
	manualset3
216059	3	419917	7	NULL	NULL	0	NULL	C = C ( 0 ) e ( - kt )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The phenanthrene biodegradation could be best described by the first order rate model , C = C ( 0 ) e ( - kt ) , where k ( the rate constant ) is equaled to 0.1185 , under the optimal condition .
	manualset3
216060	4	419917	7	NULL	NULL	0	NULL	k	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The phenanthrene biodegradation could be best described by the first order rate model , C = C ( 0 ) e ( - kt ) , where k ( the rate constant ) is equaled to 0.1185 , under the optimal condition .
	manualset3
216061	5	419917	7	NULL	NULL	0	NULL	rate constant 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The phenanthrene biodegradation could be best described by the first order rate model , C = C ( 0 ) e ( - kt ) , where k ( the rate constant ) is equaled to 0.1185 , under the optimal condition .
	manualset3
216062	6	419917	7	NULL	NULL	0	NULL	 0.1185	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The phenanthrene biodegradation could be best described by the first order rate model , C = C ( 0 ) e ( - kt ) , where k ( the rate constant ) is equaled to 0.1185 , under the optimal condition .
	manualset3
216063	7	419917	7	NULL	NULL	0	NULL	optimal condition	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The phenanthrene biodegradation could be best described by the first order rate model , C = C ( 0 ) e ( - kt ) , where k ( the rate constant ) is equaled to 0.1185 , under the optimal condition .
	manualset3
216064	1	419918	7	NULL	NULL	0	NULL	modified oligonucleotide	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The modified oligonucleotide is characterized by a chair-like structure consisting of two G-tetrads connected by three edge-wise TT , TGT and TT loops .
	manualset3
216065	2	419918	7	NULL	NULL	0	NULL	chair-like structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The modified oligonucleotide is characterized by a chair-like structure consisting of two G-tetrads connected by three edge-wise TT , TGT and TT loops .
	manualset3
216066	3	419918	7	NULL	NULL	NULL	NULL	two G-tetrads	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The modified oligonucleotide is characterized by a chair-like structure consisting of two G-tetrads connected by three edge-wise TT , TGT and TT loops .
	manualset3
216067	4	419918	7	NULL	NULL	0	NULL	three edge-wise TT loops	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The modified oligonucleotide is characterized by a chair-like structure consisting of two G-tetrads connected by three edge-wise TT , TGT and TT loops .
	manualset3
216068	5	419918	7	NULL	NULL	0	NULL	TGT loops	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The modified oligonucleotide is characterized by a chair-like structure consisting of two G-tetrads connected by three edge-wise TT , TGT and TT loops .
	manualset3
216069	6	419918	7	NULL	NULL	0	NULL	TT loops	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The modified oligonucleotide is characterized by a chair-like structure consisting of two G-tetrads connected by three edge-wise TT , TGT and TT loops .
	manualset3
216070	1	419919	7	NULL	NULL	0	NULL	Brain tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Brain tumors are the second most common malignancy of childhood after acute lymphocytic leukemia .
	manualset3
216071	2	419919	7	NULL	NULL	0	NULL	second most common malignancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Brain tumors are the second most common malignancy of childhood after acute lymphocytic leukemia .
	manualset3
216072	3	419919	7	NULL	NULL	0	NULL	childhood	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Brain tumors are the second most common malignancy of childhood after acute lymphocytic leukemia .
	manualset3
216073	4	419919	7	NULL	NULL	0	NULL	acute lymphocytic leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Brain tumors are the second most common malignancy of childhood after acute lymphocytic leukemia .
	manualset3
216074	1	419920	7	NULL	NULL	0	NULL	formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation of long-term CTA memory was dependent on the dose of LiCl paired with sucrose during acquisition .
	manualset3
216075	2	419920	7	NULL	NULL	0	NULL	long-term CTA memory	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation of long-term CTA memory was dependent on the dose of LiCl paired with sucrose during acquisition .
	manualset3
216076	3	419920	7	NULL	NULL	0	NULL	dose 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation of long-term CTA memory was dependent on the dose of LiCl paired with sucrose during acquisition .
	manualset3
216077	4	419920	7	NULL	NULL	0	NULL	LiCl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation of long-term CTA memory was dependent on the dose of LiCl paired with sucrose during acquisition .
	manualset3
216078	5	419920	7	NULL	NULL	0	NULL	sucrose	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation of long-term CTA memory was dependent on the dose of LiCl paired with sucrose during acquisition .
	manualset3
216079	6	419920	7	NULL	NULL	0	NULL	acquisition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation of long-term CTA memory was dependent on the dose of LiCl paired with sucrose during acquisition .
	manualset3
216080	1	419921	7	NULL	NULL	0	NULL	efficacy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the efficacy of DNA transfection , which is a major concern , is low in nonviral vector-mediated gene transfer compared with viral ones , nonviral vectors are relatively easy to prepare , less immunogenic and oncogenic , and have no potential of virus recombination and no limitation on the size of a transferred gene .
	manualset3
216081	2	419921	7	NULL	NULL	0	NULL	DNA transfection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the efficacy of DNA transfection , which is a major concern , is low in nonviral vector-mediated gene transfer compared with viral ones , nonviral vectors are relatively easy to prepare , less immunogenic and oncogenic , and have no potential of virus recombination and no limitation on the size of a transferred gene .
	manualset3
216082	3	419921	7	NULL	NULL	0	NULL	major concern	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the efficacy of DNA transfection , which is a major concern , is low in nonviral vector-mediated gene transfer compared with viral ones , nonviral vectors are relatively easy to prepare , less immunogenic and oncogenic , and have no potential of virus recombination and no limitation on the size of a transferred gene .
	manualset3
216083	4	419921	7	NULL	NULL	0	NULL	nonviral vector-mediated gene transfer	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the efficacy of DNA transfection , which is a major concern , is low in nonviral vector-mediated gene transfer compared with viral ones , nonviral vectors are relatively easy to prepare , less immunogenic and oncogenic , and have no potential of virus recombination and no limitation on the size of a transferred gene .
	manualset3
216084	5	419921	7	NULL	NULL	0	NULL	viral ones	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the efficacy of DNA transfection , which is a major concern , is low in nonviral vector-mediated gene transfer compared with viral ones , nonviral vectors are relatively easy to prepare , less immunogenic and oncogenic , and have no potential of virus recombination and no limitation on the size of a transferred gene .
	manualset3
216085	6	419921	7	NULL	NULL	0	NULL	nonviral vectors 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the efficacy of DNA transfection , which is a major concern , is low in nonviral vector-mediated gene transfer compared with viral ones , nonviral vectors are relatively easy to prepare , less immunogenic and oncogenic , and have no potential of virus recombination and no limitation on the size of a transferred gene .
	manualset3
216086	7	419921	7	NULL	NULL	0	NULL	virus recombination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the efficacy of DNA transfection , which is a major concern , is low in nonviral vector-mediated gene transfer compared with viral ones , nonviral vectors are relatively easy to prepare , less immunogenic and oncogenic , and have no potential of virus recombination and no limitation on the size of a transferred gene .
	manualset3
216087	8	419921	7	NULL	NULL	0	NULL	no limitation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the efficacy of DNA transfection , which is a major concern , is low in nonviral vector-mediated gene transfer compared with viral ones , nonviral vectors are relatively easy to prepare , less immunogenic and oncogenic , and have no potential of virus recombination and no limitation on the size of a transferred gene .
	manualset3
216088	9	419921	7	NULL	NULL	0	NULL	 size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the efficacy of DNA transfection , which is a major concern , is low in nonviral vector-mediated gene transfer compared with viral ones , nonviral vectors are relatively easy to prepare , less immunogenic and oncogenic , and have no potential of virus recombination and no limitation on the size of a transferred gene .
	manualset3
216089	10	419921	7	NULL	NULL	0	NULL	transferred gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the efficacy of DNA transfection , which is a major concern , is low in nonviral vector-mediated gene transfer compared with viral ones , nonviral vectors are relatively easy to prepare , less immunogenic and oncogenic , and have no potential of virus recombination and no limitation on the size of a transferred gene .
	manualset3
216090	1	419922	7	NULL	NULL	0	NULL	VDR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The VDR has a number of common polymorphisms , including a TaqI restriction fragment length polymorphism in exon 9 and a poly ( A ) length polymorphism in the 3 ' - untranslated region .
	manualset3
216091	2	419922	7	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The VDR has a number of common polymorphisms , including a TaqI restriction fragment length polymorphism in exon 9 and a poly ( A ) length polymorphism in the 3 ' - untranslated region .
	manualset3
216092	3	419922	7	NULL	NULL	NULL	NULL	common polymorphisms	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The VDR has a number of common polymorphisms , including a TaqI restriction fragment length polymorphism in exon 9 and a poly ( A ) length polymorphism in the 3 ' - untranslated region .
	manualset3
216093	4	419922	7	NULL	NULL	0	NULL	TaqI restriction fragment length polymorphism 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The VDR has a number of common polymorphisms , including a TaqI restriction fragment length polymorphism in exon 9 and a poly ( A ) length polymorphism in the 3 ' - untranslated region .
	manualset3
216094	5	419922	7	NULL	NULL	0	NULL	exon 9	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The VDR has a number of common polymorphisms , including a TaqI restriction fragment length polymorphism in exon 9 and a poly ( A ) length polymorphism in the 3 ' - untranslated region .
	manualset3
216095	6	419922	7	NULL	NULL	0	NULL	poly ( A ) length polymorphism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The VDR has a number of common polymorphisms , including a TaqI restriction fragment length polymorphism in exon 9 and a poly ( A ) length polymorphism in the 3 ' - untranslated region .
	manualset3
216096	7	419922	7	NULL	NULL	0	NULL	3 ' - untranslated region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The VDR has a number of common polymorphisms , including a TaqI restriction fragment length polymorphism in exon 9 and a poly ( A ) length polymorphism in the 3 ' - untranslated region .
	manualset3
216097	1	419923	7	NULL	NULL	0	NULL	 balloon	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	When the balloon of the autoperfusion catheter is deployed and inflated in an artery , the guide wire is removed , and the hub of the guide-wire lumen is capped .
	manualset3
216098	2	419923	7	NULL	NULL	0	NULL	autoperfusion catheter	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	When the balloon of the autoperfusion catheter is deployed and inflated in an artery , the guide wire is removed , and the hub of the guide-wire lumen is capped .
	manualset3
216099	3	419923	7	NULL	NULL	0	NULL	artery 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When the balloon of the autoperfusion catheter is deployed and inflated in an artery , the guide wire is removed , and the hub of the guide-wire lumen is capped .
	manualset3
216100	4	419923	7	NULL	NULL	0	NULL	guide wire	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	When the balloon of the autoperfusion catheter is deployed and inflated in an artery , the guide wire is removed , and the hub of the guide-wire lumen is capped .
	manualset3
216101	5	419923	7	NULL	NULL	0	NULL	 hub of the guide-wire lumen	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	When the balloon of the autoperfusion catheter is deployed and inflated in an artery , the guide wire is removed , and the hub of the guide-wire lumen is capped .
	manualset3
216102	1	419924	7	NULL	NULL	0	NULL	Study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Study of metabololic syndrome from the intrauterine growth ) .
	manualset3
216103	2	419924	7	NULL	NULL	0	NULL	metabololic syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Study of metabololic syndrome from the intrauterine growth ) .
	manualset3
216104	3	419924	7	NULL	NULL	0	NULL	intrauterine growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Study of metabololic syndrome from the intrauterine growth ) .
	manualset3
216105	1	419925	7	NULL	NULL	0	NULL	sequence 5 ' - TTTGGGGC-3 '	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	We focused on the sequence 5 ' - TTTGGGGC-3 ' ( -8 to -1 in the promoter region ) resembling the E2F binding site ( one base mismatch , TFSEARCH score 86.2 ) .
	manualset3
216106	2	419925	7	NULL	NULL	0	NULL	 -8 to -1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	We focused on the sequence 5 ' - TTTGGGGC-3 ' ( -8 to -1 in the promoter region ) resembling the E2F binding site ( one base mismatch , TFSEARCH score 86.2 ) .
	manualset3
216107	3	419925	7	NULL	NULL	0	NULL	promoter region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	We focused on the sequence 5 ' - TTTGGGGC-3 ' ( -8 to -1 in the promoter region ) resembling the E2F binding site ( one base mismatch , TFSEARCH score 86.2 ) .
	manualset3
216108	4	419925	7	NULL	NULL	0	NULL	E2F binding site	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	We focused on the sequence 5 ' - TTTGGGGC-3 ' ( -8 to -1 in the promoter region ) resembling the E2F binding site ( one base mismatch , TFSEARCH score 86.2 ) .
	manualset3
216109	5	419925	7	NULL	NULL	0	NULL	one base mismatch	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We focused on the sequence 5 ' - TTTGGGGC-3 ' ( -8 to -1 in the promoter region ) resembling the E2F binding site ( one base mismatch , TFSEARCH score 86.2 ) .
	manualset3
216110	6	419925	7	NULL	NULL	0	NULL	TFSEARCH	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We focused on the sequence 5 ' - TTTGGGGC-3 ' ( -8 to -1 in the promoter region ) resembling the E2F binding site ( one base mismatch , TFSEARCH score 86.2 ) .
	manualset3
216111	7	419925	7	NULL	NULL	0	NULL	score 86.2	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We focused on the sequence 5 ' - TTTGGGGC-3 ' ( -8 to -1 in the promoter region ) resembling the E2F binding site ( one base mismatch , TFSEARCH score 86.2 ) .
	manualset3
216112	1	419926	7	NULL	NULL	0	NULL	LOH	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	LOH for BRCA1 was detected in 18.1 % , of TP53 in 26.9 % , and of TCRD in 26.3 % of informative cases .
	manualset3
216113	2	419926	7	NULL	NULL	0	NULL	BRCA1	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	LOH for BRCA1 was detected in 18.1 % , of TP53 in 26.9 % , and of TCRD in 26.3 % of informative cases .
	manualset3
216114	3	419926	7	NULL	NULL	0	NULL	18.1 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	LOH for BRCA1 was detected in 18.1 % , of TP53 in 26.9 % , and of TCRD in 26.3 % of informative cases .
	manualset3
216115	4	419926	7	NULL	NULL	0	NULL	TP53	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	LOH for BRCA1 was detected in 18.1 % , of TP53 in 26.9 % , and of TCRD in 26.3 % of informative cases .
	manualset3
216116	5	419926	7	NULL	NULL	0	NULL	26.9 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	LOH for BRCA1 was detected in 18.1 % , of TP53 in 26.9 % , and of TCRD in 26.3 % of informative cases .
	manualset3
216117	6	419926	7	NULL	NULL	0	NULL	 TCRD	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	LOH for BRCA1 was detected in 18.1 % , of TP53 in 26.9 % , and of TCRD in 26.3 % of informative cases .
	manualset3
216118	7	419926	7	NULL	NULL	0	NULL	26.3 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	LOH for BRCA1 was detected in 18.1 % , of TP53 in 26.9 % , and of TCRD in 26.3 % of informative cases .
	manualset3
216119	8	419926	7	NULL	NULL	0	NULL	informative cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	LOH for BRCA1 was detected in 18.1 % , of TP53 in 26.9 % , and of TCRD in 26.3 % of informative cases .
	manualset3
216120	1	419927	7	NULL	NULL	0	NULL	survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The survival of H. microstoma was affected only when rejection of T. spiralis coincided with the intestinal phase of the cestode : if T. spiralis rejection was timed to occur after the scolex of the cestode had entered the bile duct there was no loss of H. microstoma .
	manualset3
216121	2	419927	7	NULL	NULL	0	NULL	H. microstoma	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The survival of H. microstoma was affected only when rejection of T. spiralis coincided with the intestinal phase of the cestode : if T. spiralis rejection was timed to occur after the scolex of the cestode had entered the bile duct there was no loss of H. microstoma .
	manualset3
216122	3	419927	7	NULL	NULL	0	NULL	rejection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The survival of H. microstoma was affected only when rejection of T. spiralis coincided with the intestinal phase of the cestode : if T. spiralis rejection was timed to occur after the scolex of the cestode had entered the bile duct there was no loss of H. microstoma .
	manualset3
216123	4	419927	7	NULL	NULL	0	NULL	T. spiralis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The survival of H. microstoma was affected only when rejection of T. spiralis coincided with the intestinal phase of the cestode : if T. spiralis rejection was timed to occur after the scolex of the cestode had entered the bile duct there was no loss of H. microstoma .
	manualset3
216124	5	419927	7	NULL	NULL	0	NULL	 intestinal phase	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The survival of H. microstoma was affected only when rejection of T. spiralis coincided with the intestinal phase of the cestode : if T. spiralis rejection was timed to occur after the scolex of the cestode had entered the bile duct there was no loss of H. microstoma .
	manualset3
216125	6	419927	7	NULL	NULL	0	NULL	cestode	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The survival of H. microstoma was affected only when rejection of T. spiralis coincided with the intestinal phase of the cestode : if T. spiralis rejection was timed to occur after the scolex of the cestode had entered the bile duct there was no loss of H. microstoma .
	manualset3
216126	7	419927	7	NULL	NULL	0	NULL	T. spiralis rejection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The survival of H. microstoma was affected only when rejection of T. spiralis coincided with the intestinal phase of the cestode : if T. spiralis rejection was timed to occur after the scolex of the cestode had entered the bile duct there was no loss of H. microstoma .
	manualset3
216127	8	419927	7	NULL	NULL	0	NULL	scolex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The survival of H. microstoma was affected only when rejection of T. spiralis coincided with the intestinal phase of the cestode : if T. spiralis rejection was timed to occur after the scolex of the cestode had entered the bile duct there was no loss of H. microstoma .
	manualset3
216128	9	419927	7	NULL	NULL	0	NULL	cestode	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The survival of H. microstoma was affected only when rejection of T. spiralis coincided with the intestinal phase of the cestode : if T. spiralis rejection was timed to occur after the scolex of the cestode had entered the bile duct there was no loss of H. microstoma .
	manualset3
216129	10	419927	7	NULL	NULL	0	NULL	bile duct	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The survival of H. microstoma was affected only when rejection of T. spiralis coincided with the intestinal phase of the cestode : if T. spiralis rejection was timed to occur after the scolex of the cestode had entered the bile duct there was no loss of H. microstoma .
	manualset3
216130	11	419927	7	NULL	NULL	0	NULL	no loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The survival of H. microstoma was affected only when rejection of T. spiralis coincided with the intestinal phase of the cestode : if T. spiralis rejection was timed to occur after the scolex of the cestode had entered the bile duct there was no loss of H. microstoma .
	manualset3
216131	12	419927	7	NULL	NULL	0	NULL	H. microstoma	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The survival of H. microstoma was affected only when rejection of T. spiralis coincided with the intestinal phase of the cestode : if T. spiralis rejection was timed to occur after the scolex of the cestode had entered the bile duct there was no loss of H. microstoma .
	manualset3
216132	1	419928	7	NULL	NULL	0	NULL	alcoholic extract	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An alcoholic extract of aerial parts of C. decidua , including flowers and fruits , was screened for central nervous system ( CNS ) activity using conventional behavioral animal models .
	manualset3
216133	2	419928	7	NULL	NULL	0	NULL	aerial parts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An alcoholic extract of aerial parts of C. decidua , including flowers and fruits , was screened for central nervous system ( CNS ) activity using conventional behavioral animal models .
	manualset3
216134	3	419928	7	NULL	NULL	0	NULL	C. decidua	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	An alcoholic extract of aerial parts of C. decidua , including flowers and fruits , was screened for central nervous system ( CNS ) activity using conventional behavioral animal models .
	manualset3
216135	4	419928	7	NULL	NULL	0	NULL	flowers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An alcoholic extract of aerial parts of C. decidua , including flowers and fruits , was screened for central nervous system ( CNS ) activity using conventional behavioral animal models .
	manualset3
216136	5	419928	7	NULL	NULL	NULL	NULL	 fruits	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An alcoholic extract of aerial parts of C. decidua , including flowers and fruits , was screened for central nervous system ( CNS ) activity using conventional behavioral animal models .
	manualset3
216137	6	419928	7	NULL	NULL	0	NULL	central nervous system ( CNS ) activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An alcoholic extract of aerial parts of C. decidua , including flowers and fruits , was screened for central nervous system ( CNS ) activity using conventional behavioral animal models .
	manualset3
216138	7	419928	7	NULL	NULL	0	NULL	conventional behavioral animal models	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	An alcoholic extract of aerial parts of C. decidua , including flowers and fruits , was screened for central nervous system ( CNS ) activity using conventional behavioral animal models .
	manualset3
216139	1	419929	7	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In both cases , spinal T2-weighted magnetic resonance images showed edema of the spinal cord , indicating a flow void around it .
	manualset3
216140	2	419929	7	NULL	NULL	0	NULL	spinal T2-weighted magnetic resonance images	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In both cases , spinal T2-weighted magnetic resonance images showed edema of the spinal cord , indicating a flow void around it .
	manualset3
216141	3	419929	7	NULL	NULL	0	NULL	edema	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In both cases , spinal T2-weighted magnetic resonance images showed edema of the spinal cord , indicating a flow void around it .
	manualset3
216142	4	419929	7	NULL	NULL	0	NULL	spinal cord	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In both cases , spinal T2-weighted magnetic resonance images showed edema of the spinal cord , indicating a flow void around it .
	manualset3
216143	5	419929	7	NULL	NULL	0	NULL	flow void	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In both cases , spinal T2-weighted magnetic resonance images showed edema of the spinal cord , indicating a flow void around it .
	manualset3
216144	1	419930	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These and other results ( e.g. , proteinase inhibitor profiling ) indicate that ovine skeletal muscle does indeed contain MCP and that its biochemical properties are the same as MCP isolated from other sources .
	manualset3
216145	2	419930	7	NULL	NULL	0	NULL	proteinase inhibitor profiling	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These and other results ( e.g. , proteinase inhibitor profiling ) indicate that ovine skeletal muscle does indeed contain MCP and that its biochemical properties are the same as MCP isolated from other sources .
	manualset3
216146	3	419930	7	NULL	NULL	0	NULL	ovine skeletal muscle 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These and other results ( e.g. , proteinase inhibitor profiling ) indicate that ovine skeletal muscle does indeed contain MCP and that its biochemical properties are the same as MCP isolated from other sources .
	manualset3
216147	4	419930	7	NULL	NULL	0	NULL	 MCP	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These and other results ( e.g. , proteinase inhibitor profiling ) indicate that ovine skeletal muscle does indeed contain MCP and that its biochemical properties are the same as MCP isolated from other sources .
	manualset3
216148	5	419930	7	NULL	NULL	0	NULL	biochemical properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These and other results ( e.g. , proteinase inhibitor profiling ) indicate that ovine skeletal muscle does indeed contain MCP and that its biochemical properties are the same as MCP isolated from other sources .
	manualset3
216149	6	419930	7	NULL	NULL	0	NULL	MCP	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These and other results ( e.g. , proteinase inhibitor profiling ) indicate that ovine skeletal muscle does indeed contain MCP and that its biochemical properties are the same as MCP isolated from other sources .
	manualset3
216150	7	419930	7	NULL	NULL	0	NULL	 sources	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These and other results ( e.g. , proteinase inhibitor profiling ) indicate that ovine skeletal muscle does indeed contain MCP and that its biochemical properties are the same as MCP isolated from other sources .
	manualset3
216153	1	419931	7	NULL	NULL	0	NULL	enzyme 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the enzyme was previously thought to be entirely cytosolic , digitonin fractionation has shown that a portion of total cellular ATP citrate lyase is bound to mitochondria or some other structure , and the amount bound varies with the animal 's nutritional state .
	manualset3
216154	2	419931	7	NULL	NULL	0	NULL	digitonin fractionation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the enzyme was previously thought to be entirely cytosolic , digitonin fractionation has shown that a portion of total cellular ATP citrate lyase is bound to mitochondria or some other structure , and the amount bound varies with the animal 's nutritional state .
	manualset3
216155	3	419931	7	NULL	NULL	0	NULL	portion 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the enzyme was previously thought to be entirely cytosolic , digitonin fractionation has shown that a portion of total cellular ATP citrate lyase is bound to mitochondria or some other structure , and the amount bound varies with the animal 's nutritional state .
	manualset3
216156	4	419931	7	NULL	NULL	0	NULL	total cellular ATP citrate lyase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the enzyme was previously thought to be entirely cytosolic , digitonin fractionation has shown that a portion of total cellular ATP citrate lyase is bound to mitochondria or some other structure , and the amount bound varies with the animal 's nutritional state .
	manualset3
216157	5	419931	7	NULL	NULL	0	NULL	mitochondria 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the enzyme was previously thought to be entirely cytosolic , digitonin fractionation has shown that a portion of total cellular ATP citrate lyase is bound to mitochondria or some other structure , and the amount bound varies with the animal 's nutritional state .
	manualset3
216158	6	419931	7	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the enzyme was previously thought to be entirely cytosolic , digitonin fractionation has shown that a portion of total cellular ATP citrate lyase is bound to mitochondria or some other structure , and the amount bound varies with the animal 's nutritional state .
	manualset3
216159	7	419931	7	NULL	NULL	0	NULL	animal 's nutritional state	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the enzyme was previously thought to be entirely cytosolic , digitonin fractionation has shown that a portion of total cellular ATP citrate lyase is bound to mitochondria or some other structure , and the amount bound varies with the animal 's nutritional state .
	manualset3
217438	8	419931	7	NULL	NULL	0	NULL	structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the enzyme was previously thought to be entirely cytosolic , digitonin fractionation has shown that a portion of total cellular ATP citrate lyase is bound to mitochondria or some other structure , and the amount bound varies with the animal 's nutritional state .
	manualset3
216160	1	419932	7	NULL	NULL	0	NULL	Effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of lipid-lowering pharmaceuticals bezafibrate and clofibric acid on lipid metabolism in fathead minnow ( Pimephales promelas ) .
	manualset3
216161	2	419932	7	NULL	NULL	0	NULL	lipid-lowering pharmaceuticals 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of lipid-lowering pharmaceuticals bezafibrate and clofibric acid on lipid metabolism in fathead minnow ( Pimephales promelas ) .
	manualset3
216162	3	419932	7	NULL	NULL	NULL	NULL	bezafibrate 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effects of lipid-lowering pharmaceuticals bezafibrate and clofibric acid on lipid metabolism in fathead minnow ( Pimephales promelas ) .
	manualset3
216163	4	419932	7	NULL	NULL	0	NULL	clofibric acid	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of lipid-lowering pharmaceuticals bezafibrate and clofibric acid on lipid metabolism in fathead minnow ( Pimephales promelas ) .
	manualset3
216164	5	419932	7	NULL	NULL	0	NULL	lipid metabolism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of lipid-lowering pharmaceuticals bezafibrate and clofibric acid on lipid metabolism in fathead minnow ( Pimephales promelas ) .
	manualset3
216165	6	419932	7	NULL	NULL	0	NULL	fathead minnow	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of lipid-lowering pharmaceuticals bezafibrate and clofibric acid on lipid metabolism in fathead minnow ( Pimephales promelas ) .
	manualset3
216166	7	419932	7	NULL	NULL	0	NULL	Pimephales promelas 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of lipid-lowering pharmaceuticals bezafibrate and clofibric acid on lipid metabolism in fathead minnow ( Pimephales promelas ) .
	manualset3
216167	1	419933	7	NULL	NULL	0	NULL	Structural study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural study of the alpha chain of one hemoglobin from the adults salamander , Pleurodeles waltlii .
	manualset3
216168	2	419933	7	NULL	NULL	0	NULL	alpha chain 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural study of the alpha chain of one hemoglobin from the adults salamander , Pleurodeles waltlii .
	manualset3
216169	3	419933	7	NULL	NULL	0	NULL	one hemoglobin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural study of the alpha chain of one hemoglobin from the adults salamander , Pleurodeles waltlii .
	manualset3
216170	4	419933	7	NULL	NULL	0	NULL	adults salamander	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural study of the alpha chain of one hemoglobin from the adults salamander , Pleurodeles waltlii .
	manualset3
216171	5	419933	7	NULL	NULL	0	NULL	Pleurodeles waltlii	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural study of the alpha chain of one hemoglobin from the adults salamander , Pleurodeles waltlii .
	manualset3
216172	1	419934	7	NULL	NULL	0	NULL	 tripartite CAK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This tripartite CAK occurs in a free form and in association with ` core ' TFIIH , which functions in both pol II transcription and DNA repair .
	manualset3
216173	2	419934	7	NULL	NULL	0	NULL	 free form 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This tripartite CAK occurs in a free form and in association with ` core ' TFIIH , which functions in both pol II transcription and DNA repair .
	manualset3
216174	3	419934	7	NULL	NULL	0	NULL	 ` core ' TFIIH 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This tripartite CAK occurs in a free form and in association with ` core ' TFIIH , which functions in both pol II transcription and DNA repair .
	manualset3
216175	4	419934	7	NULL	NULL	0	NULL	pol II transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This tripartite CAK occurs in a free form and in association with ` core ' TFIIH , which functions in both pol II transcription and DNA repair .
	manualset3
216176	5	419934	7	NULL	NULL	0	NULL	DNA repair 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This tripartite CAK occurs in a free form and in association with ` core ' TFIIH , which functions in both pol II transcription and DNA repair .
	manualset3
216177	1	419935	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support an interpretation of CYS3 as a transcriptional activator whose regulation is a crucial control point in the signal response pathway triggered by sulfur limitation .
	manualset3
216178	2	419935	7	NULL	NULL	0	NULL	interpretation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support an interpretation of CYS3 as a transcriptional activator whose regulation is a crucial control point in the signal response pathway triggered by sulfur limitation .
	manualset3
216179	3	419935	7	NULL	NULL	0	NULL	CYS3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support an interpretation of CYS3 as a transcriptional activator whose regulation is a crucial control point in the signal response pathway triggered by sulfur limitation .
	manualset3
216180	4	419935	7	NULL	NULL	0	NULL	 transcriptional activator	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support an interpretation of CYS3 as a transcriptional activator whose regulation is a crucial control point in the signal response pathway triggered by sulfur limitation .
	manualset3
216181	5	419935	7	NULL	NULL	0	NULL	regulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support an interpretation of CYS3 as a transcriptional activator whose regulation is a crucial control point in the signal response pathway triggered by sulfur limitation .
	manualset3
216182	6	419935	7	NULL	NULL	0	NULL	crucial control point 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support an interpretation of CYS3 as a transcriptional activator whose regulation is a crucial control point in the signal response pathway triggered by sulfur limitation .
	manualset3
216183	7	419935	7	NULL	NULL	0	NULL	signal response pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support an interpretation of CYS3 as a transcriptional activator whose regulation is a crucial control point in the signal response pathway triggered by sulfur limitation .
	manualset3
216184	8	419935	7	NULL	NULL	0	NULL	 sulfur limitation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results support an interpretation of CYS3 as a transcriptional activator whose regulation is a crucial control point in the signal response pathway triggered by sulfur limitation .
	manualset3
216185	1	419936	7	NULL	NULL	0	NULL	simplified version	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To improve efficiency further a simplified version of this estimate was devised and validated on carcinoma cell nuclei in 200 fields ( 20 sets of 10 ) selected from 20 invasive cervical carcinomas .
	manualset3
216186	2	419936	7	NULL	NULL	0	NULL	estimate 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To improve efficiency further a simplified version of this estimate was devised and validated on carcinoma cell nuclei in 200 fields ( 20 sets of 10 ) selected from 20 invasive cervical carcinomas .
	manualset3
216187	3	419936	7	NULL	NULL	0	NULL	carcinoma cell nuclei 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	To improve efficiency further a simplified version of this estimate was devised and validated on carcinoma cell nuclei in 200 fields ( 20 sets of 10 ) selected from 20 invasive cervical carcinomas .
	manualset3
216188	4	419936	7	NULL	NULL	0	NULL	200 fields	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To improve efficiency further a simplified version of this estimate was devised and validated on carcinoma cell nuclei in 200 fields ( 20 sets of 10 ) selected from 20 invasive cervical carcinomas .
	manualset3
216189	5	419936	7	NULL	NULL	0	NULL	20 sets of 10	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To improve efficiency further a simplified version of this estimate was devised and validated on carcinoma cell nuclei in 200 fields ( 20 sets of 10 ) selected from 20 invasive cervical carcinomas .
	manualset3
216190	6	419936	7	NULL	NULL	0	NULL	20 invasive cervical carcinomas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To improve efficiency further a simplified version of this estimate was devised and validated on carcinoma cell nuclei in 200 fields ( 20 sets of 10 ) selected from 20 invasive cervical carcinomas .
	manualset3
216191	1	419937	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data support the hypothesis that localized persistent infection may influence systemic levels of inflammatory mediators .
	manualset3
216192	2	419937	7	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The data support the hypothesis that localized persistent infection may influence systemic levels of inflammatory mediators .
	manualset3
216193	3	419937	7	NULL	NULL	0	NULL	localized persistent infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The data support the hypothesis that localized persistent infection may influence systemic levels of inflammatory mediators .
	manualset3
216194	4	419937	7	NULL	NULL	0	NULL	systemic levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data support the hypothesis that localized persistent infection may influence systemic levels of inflammatory mediators .
	manualset3
216195	5	419937	7	NULL	NULL	0	NULL	inflammatory mediators	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The data support the hypothesis that localized persistent infection may influence systemic levels of inflammatory mediators .
	manualset3
216196	1	419938	7	NULL	NULL	0	NULL	Interocular transfer	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Interocular transfer of adaptation after effect in neurons of area 17 and 18 of split chiasm cats .
	manualset3
216197	2	419938	7	NULL	NULL	NULL	NULL	adaptation after effect	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Interocular transfer of adaptation after effect in neurons of area 17 and 18 of split chiasm cats .
	manualset3
216198	3	419938	7	NULL	NULL	0	NULL	neurons	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Interocular transfer of adaptation after effect in neurons of area 17 and 18 of split chiasm cats .
	manualset3
216199	4	419938	7	NULL	NULL	NULL	NULL	area 17	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Interocular transfer of adaptation after effect in neurons of area 17 and 18 of split chiasm cats .
	manualset3
216200	5	419938	7	NULL	NULL	NULL	NULL	area 18	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Interocular transfer of adaptation after effect in neurons of area 17 and 18 of split chiasm cats .
	manualset3
216201	6	419938	7	NULL	NULL	0	NULL	split chiasm cats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Interocular transfer of adaptation after effect in neurons of area 17 and 18 of split chiasm cats .
	manualset3
216202	1	419939	7	NULL	NULL	0	NULL	flat culture 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the flat culture was useful for the induction of somites and of neural plates , we describe the advantages of culture without the area opaca of neural plates induced by tubulin mRNA or by TPA , which can differentiate into neural tubes .
	manualset3
216203	2	419939	7	NULL	NULL	0	NULL	induction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the flat culture was useful for the induction of somites and of neural plates , we describe the advantages of culture without the area opaca of neural plates induced by tubulin mRNA or by TPA , which can differentiate into neural tubes .
	manualset3
216204	3	419939	7	NULL	NULL	0	NULL	somites	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the flat culture was useful for the induction of somites and of neural plates , we describe the advantages of culture without the area opaca of neural plates induced by tubulin mRNA or by TPA , which can differentiate into neural tubes .
	manualset3
216205	4	419939	7	NULL	NULL	0	NULL	 neural plates	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the flat culture was useful for the induction of somites and of neural plates , we describe the advantages of culture without the area opaca of neural plates induced by tubulin mRNA or by TPA , which can differentiate into neural tubes .
	manualset3
216206	5	419939	7	NULL	NULL	0	NULL	advantages	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the flat culture was useful for the induction of somites and of neural plates , we describe the advantages of culture without the area opaca of neural plates induced by tubulin mRNA or by TPA , which can differentiate into neural tubes .
	manualset3
216207	6	419939	7	NULL	NULL	0	NULL	culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the flat culture was useful for the induction of somites and of neural plates , we describe the advantages of culture without the area opaca of neural plates induced by tubulin mRNA or by TPA , which can differentiate into neural tubes .
	manualset3
216208	7	419939	7	NULL	NULL	0	NULL	area opaca	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the flat culture was useful for the induction of somites and of neural plates , we describe the advantages of culture without the area opaca of neural plates induced by tubulin mRNA or by TPA , which can differentiate into neural tubes .
	manualset3
216209	8	419939	7	NULL	NULL	0	NULL	neural plates	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the flat culture was useful for the induction of somites and of neural plates , we describe the advantages of culture without the area opaca of neural plates induced by tubulin mRNA or by TPA , which can differentiate into neural tubes .
	manualset3
216210	9	419939	7	NULL	NULL	0	NULL	tubulin mRNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the flat culture was useful for the induction of somites and of neural plates , we describe the advantages of culture without the area opaca of neural plates induced by tubulin mRNA or by TPA , which can differentiate into neural tubes .
	manualset3
216211	10	419939	7	NULL	NULL	0	NULL	TPA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the flat culture was useful for the induction of somites and of neural plates , we describe the advantages of culture without the area opaca of neural plates induced by tubulin mRNA or by TPA , which can differentiate into neural tubes .
	manualset3
216212	11	419939	7	NULL	NULL	0	NULL	neural tubes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the flat culture was useful for the induction of somites and of neural plates , we describe the advantages of culture without the area opaca of neural plates induced by tubulin mRNA or by TPA , which can differentiate into neural tubes .
	manualset3
216213	1	419940	7	NULL	NULL	0	NULL	Allyl alcohol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Allyl alcohol was not mutagenic in four strains of S. typhimurium , with or without S9 metabolic activation .
	manualset3
216214	2	419940	7	NULL	NULL	0	NULL	four strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Allyl alcohol was not mutagenic in four strains of S. typhimurium , with or without S9 metabolic activation .
	manualset3
216215	3	419940	7	NULL	NULL	0	NULL	S. typhimurium	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Allyl alcohol was not mutagenic in four strains of S. typhimurium , with or without S9 metabolic activation .
	manualset3
216216	4	419940	7	NULL	NULL	0	NULL	S9 metabolic activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Allyl alcohol was not mutagenic in four strains of S. typhimurium , with or without S9 metabolic activation .
	manualset3
216217	1	419941	7	NULL	NULL	0	NULL	calcitriol-mediated differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After calcitriol-mediated differentiation ( 72 h , measured by CD 14 expression ) mRNA expression was further enhanced by PMA ( 45-fold ) , dexamethasone ( 15-fold ) , oestradiol ( 3.7-fold ) , testosterone ( 2.5-fold ) and androstenedione ( 3.5-fold ) .
	manualset3
216218	2	419941	7	NULL	NULL	0	NULL	72 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After calcitriol-mediated differentiation ( 72 h , measured by CD 14 expression ) mRNA expression was further enhanced by PMA ( 45-fold ) , dexamethasone ( 15-fold ) , oestradiol ( 3.7-fold ) , testosterone ( 2.5-fold ) and androstenedione ( 3.5-fold ) .
	manualset3
216219	3	419941	7	NULL	NULL	0	NULL	CD 14 expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After calcitriol-mediated differentiation ( 72 h , measured by CD 14 expression ) mRNA expression was further enhanced by PMA ( 45-fold ) , dexamethasone ( 15-fold ) , oestradiol ( 3.7-fold ) , testosterone ( 2.5-fold ) and androstenedione ( 3.5-fold ) .
	manualset3
216220	4	419941	7	NULL	NULL	0	NULL	mRNA expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After calcitriol-mediated differentiation ( 72 h , measured by CD 14 expression ) mRNA expression was further enhanced by PMA ( 45-fold ) , dexamethasone ( 15-fold ) , oestradiol ( 3.7-fold ) , testosterone ( 2.5-fold ) and androstenedione ( 3.5-fold ) .
	manualset3
216221	5	419941	7	NULL	NULL	0	NULL	PMA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After calcitriol-mediated differentiation ( 72 h , measured by CD 14 expression ) mRNA expression was further enhanced by PMA ( 45-fold ) , dexamethasone ( 15-fold ) , oestradiol ( 3.7-fold ) , testosterone ( 2.5-fold ) and androstenedione ( 3.5-fold ) .
	manualset3
216222	6	419941	7	NULL	NULL	0	NULL	45-fold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After calcitriol-mediated differentiation ( 72 h , measured by CD 14 expression ) mRNA expression was further enhanced by PMA ( 45-fold ) , dexamethasone ( 15-fold ) , oestradiol ( 3.7-fold ) , testosterone ( 2.5-fold ) and androstenedione ( 3.5-fold ) .
	manualset3
216223	7	419941	7	NULL	NULL	0	NULL	 dexamethasone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	After calcitriol-mediated differentiation ( 72 h , measured by CD 14 expression ) mRNA expression was further enhanced by PMA ( 45-fold ) , dexamethasone ( 15-fold ) , oestradiol ( 3.7-fold ) , testosterone ( 2.5-fold ) and androstenedione ( 3.5-fold ) .
	manualset3
216224	8	419941	7	NULL	NULL	0	NULL	15-fold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After calcitriol-mediated differentiation ( 72 h , measured by CD 14 expression ) mRNA expression was further enhanced by PMA ( 45-fold ) , dexamethasone ( 15-fold ) , oestradiol ( 3.7-fold ) , testosterone ( 2.5-fold ) and androstenedione ( 3.5-fold ) .
	manualset3
216225	9	419941	7	NULL	NULL	0	NULL	oestradiol 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After calcitriol-mediated differentiation ( 72 h , measured by CD 14 expression ) mRNA expression was further enhanced by PMA ( 45-fold ) , dexamethasone ( 15-fold ) , oestradiol ( 3.7-fold ) , testosterone ( 2.5-fold ) and androstenedione ( 3.5-fold ) .
	manualset3
216226	10	419941	7	NULL	NULL	0	NULL	3.7-fold 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After calcitriol-mediated differentiation ( 72 h , measured by CD 14 expression ) mRNA expression was further enhanced by PMA ( 45-fold ) , dexamethasone ( 15-fold ) , oestradiol ( 3.7-fold ) , testosterone ( 2.5-fold ) and androstenedione ( 3.5-fold ) .
	manualset3
216227	11	419941	7	NULL	NULL	0	NULL	testosterone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After calcitriol-mediated differentiation ( 72 h , measured by CD 14 expression ) mRNA expression was further enhanced by PMA ( 45-fold ) , dexamethasone ( 15-fold ) , oestradiol ( 3.7-fold ) , testosterone ( 2.5-fold ) and androstenedione ( 3.5-fold ) .
	manualset3
216228	12	419941	7	NULL	NULL	0	NULL	 2.5-fold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After calcitriol-mediated differentiation ( 72 h , measured by CD 14 expression ) mRNA expression was further enhanced by PMA ( 45-fold ) , dexamethasone ( 15-fold ) , oestradiol ( 3.7-fold ) , testosterone ( 2.5-fold ) and androstenedione ( 3.5-fold ) .
	manualset3
216229	13	419941	7	NULL	NULL	NULL	NULL	androstenedione 	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	After calcitriol-mediated differentiation ( 72 h , measured by CD 14 expression ) mRNA expression was further enhanced by PMA ( 45-fold ) , dexamethasone ( 15-fold ) , oestradiol ( 3.7-fold ) , testosterone ( 2.5-fold ) and androstenedione ( 3.5-fold ) .
	manualset3
216230	14	419941	7	NULL	NULL	0	NULL	 3.5-fold 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After calcitriol-mediated differentiation ( 72 h , measured by CD 14 expression ) mRNA expression was further enhanced by PMA ( 45-fold ) , dexamethasone ( 15-fold ) , oestradiol ( 3.7-fold ) , testosterone ( 2.5-fold ) and androstenedione ( 3.5-fold ) .
	manualset3
216231	1	419942	7	NULL	NULL	0	NULL	 protein product	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed the protein product on these cultured cells by immunocytochemistry using an antibody to IFNGR .
	manualset3
216232	2	419942	7	NULL	NULL	0	NULL	cultured cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed the protein product on these cultured cells by immunocytochemistry using an antibody to IFNGR .
	manualset3
216233	3	419942	7	NULL	NULL	0	NULL	immunocytochemistry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed the protein product on these cultured cells by immunocytochemistry using an antibody to IFNGR .
	manualset3
216234	4	419942	7	NULL	NULL	0	NULL	antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed the protein product on these cultured cells by immunocytochemistry using an antibody to IFNGR .
	manualset3
216235	5	419942	7	NULL	NULL	0	NULL	IFNGR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We showed the protein product on these cultured cells by immunocytochemistry using an antibody to IFNGR .
	manualset3
216236	1	419943	7	NULL	NULL	0	NULL	significance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To assess the significance of radiographic signs of sclerosis of the third carpal bone ( C3 ) in young Standardbred trotters in relation to performance , lameness and bone turnover both carpi in 14 Standardbred trotters were radiographically and scintigraphically examined 6 times , from the beginning of speed training until the beginning of racing , between the mean ages of 20 and 42 months .
	manualset3
216237	2	419943	7	NULL	NULL	0	NULL	radiographic signs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To assess the significance of radiographic signs of sclerosis of the third carpal bone ( C3 ) in young Standardbred trotters in relation to performance , lameness and bone turnover both carpi in 14 Standardbred trotters were radiographically and scintigraphically examined 6 times , from the beginning of speed training until the beginning of racing , between the mean ages of 20 and 42 months .
	manualset3
216238	3	419943	7	NULL	NULL	0	NULL	sclerosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To assess the significance of radiographic signs of sclerosis of the third carpal bone ( C3 ) in young Standardbred trotters in relation to performance , lameness and bone turnover both carpi in 14 Standardbred trotters were radiographically and scintigraphically examined 6 times , from the beginning of speed training until the beginning of racing , between the mean ages of 20 and 42 months .
	manualset3
216239	4	419943	7	NULL	NULL	0	NULL	third carpal bone ( C3 )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To assess the significance of radiographic signs of sclerosis of the third carpal bone ( C3 ) in young Standardbred trotters in relation to performance , lameness and bone turnover both carpi in 14 Standardbred trotters were radiographically and scintigraphically examined 6 times , from the beginning of speed training until the beginning of racing , between the mean ages of 20 and 42 months .
	manualset3
216240	5	419943	7	NULL	NULL	NULL	NULL	young Standardbred trotters	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To assess the significance of radiographic signs of sclerosis of the third carpal bone ( C3 ) in young Standardbred trotters in relation to performance , lameness and bone turnover both carpi in 14 Standardbred trotters were radiographically and scintigraphically examined 6 times , from the beginning of speed training until the beginning of racing , between the mean ages of 20 and 42 months .
	manualset3
216241	6	419943	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	To assess the significance of radiographic signs of sclerosis of the third carpal bone ( C3 ) in young Standardbred trotters in relation to performance , lameness and bone turnover both carpi in 14 Standardbred trotters were radiographically and scintigraphically examined 6 times , from the beginning of speed training until the beginning of racing , between the mean ages of 20 and 42 months .
	manualset3
216242	7	419943	7	NULL	NULL	0	NULL	performance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To assess the significance of radiographic signs of sclerosis of the third carpal bone ( C3 ) in young Standardbred trotters in relation to performance , lameness and bone turnover both carpi in 14 Standardbred trotters were radiographically and scintigraphically examined 6 times , from the beginning of speed training until the beginning of racing , between the mean ages of 20 and 42 months .
	manualset3
216243	8	419943	7	NULL	NULL	0	NULL	lameness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To assess the significance of radiographic signs of sclerosis of the third carpal bone ( C3 ) in young Standardbred trotters in relation to performance , lameness and bone turnover both carpi in 14 Standardbred trotters were radiographically and scintigraphically examined 6 times , from the beginning of speed training until the beginning of racing , between the mean ages of 20 and 42 months .
	manualset3
216244	9	419943	7	NULL	NULL	0	NULL	bone turnover	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To assess the significance of radiographic signs of sclerosis of the third carpal bone ( C3 ) in young Standardbred trotters in relation to performance , lameness and bone turnover both carpi in 14 Standardbred trotters were radiographically and scintigraphically examined 6 times , from the beginning of speed training until the beginning of racing , between the mean ages of 20 and 42 months .
	manualset3
216245	10	419943	7	NULL	NULL	0	NULL	carpi	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To assess the significance of radiographic signs of sclerosis of the third carpal bone ( C3 ) in young Standardbred trotters in relation to performance , lameness and bone turnover both carpi in 14 Standardbred trotters were radiographically and scintigraphically examined 6 times , from the beginning of speed training until the beginning of racing , between the mean ages of 20 and 42 months .
	manualset3
216246	11	419943	7	NULL	NULL	0	NULL	14 Standardbred trotters	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To assess the significance of radiographic signs of sclerosis of the third carpal bone ( C3 ) in young Standardbred trotters in relation to performance , lameness and bone turnover both carpi in 14 Standardbred trotters were radiographically and scintigraphically examined 6 times , from the beginning of speed training until the beginning of racing , between the mean ages of 20 and 42 months .
	manualset3
216247	12	419943	7	NULL	NULL	0	NULL	 6 times	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To assess the significance of radiographic signs of sclerosis of the third carpal bone ( C3 ) in young Standardbred trotters in relation to performance , lameness and bone turnover both carpi in 14 Standardbred trotters were radiographically and scintigraphically examined 6 times , from the beginning of speed training until the beginning of racing , between the mean ages of 20 and 42 months .
	manualset3
216248	13	419943	7	NULL	NULL	0	NULL	beginning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To assess the significance of radiographic signs of sclerosis of the third carpal bone ( C3 ) in young Standardbred trotters in relation to performance , lameness and bone turnover both carpi in 14 Standardbred trotters were radiographically and scintigraphically examined 6 times , from the beginning of speed training until the beginning of racing , between the mean ages of 20 and 42 months .
	manualset3
216249	14	419943	7	NULL	NULL	0	NULL	speed training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To assess the significance of radiographic signs of sclerosis of the third carpal bone ( C3 ) in young Standardbred trotters in relation to performance , lameness and bone turnover both carpi in 14 Standardbred trotters were radiographically and scintigraphically examined 6 times , from the beginning of speed training until the beginning of racing , between the mean ages of 20 and 42 months .
	manualset3
216250	15	419943	7	NULL	NULL	0	NULL	beginning 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To assess the significance of radiographic signs of sclerosis of the third carpal bone ( C3 ) in young Standardbred trotters in relation to performance , lameness and bone turnover both carpi in 14 Standardbred trotters were radiographically and scintigraphically examined 6 times , from the beginning of speed training until the beginning of racing , between the mean ages of 20 and 42 months .
	manualset3
216251	16	419943	7	NULL	NULL	0	NULL	racing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To assess the significance of radiographic signs of sclerosis of the third carpal bone ( C3 ) in young Standardbred trotters in relation to performance , lameness and bone turnover both carpi in 14 Standardbred trotters were radiographically and scintigraphically examined 6 times , from the beginning of speed training until the beginning of racing , between the mean ages of 20 and 42 months .
	manualset3
216252	17	419943	7	NULL	NULL	0	NULL	mean ages	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	To assess the significance of radiographic signs of sclerosis of the third carpal bone ( C3 ) in young Standardbred trotters in relation to performance , lameness and bone turnover both carpi in 14 Standardbred trotters were radiographically and scintigraphically examined 6 times , from the beginning of speed training until the beginning of racing , between the mean ages of 20 and 42 months .
	manualset3
216253	18	419943	7	NULL	NULL	0	NULL	20 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	To assess the significance of radiographic signs of sclerosis of the third carpal bone ( C3 ) in young Standardbred trotters in relation to performance , lameness and bone turnover both carpi in 14 Standardbred trotters were radiographically and scintigraphically examined 6 times , from the beginning of speed training until the beginning of racing , between the mean ages of 20 and 42 months .
	manualset3
216254	19	419943	7	NULL	NULL	0	NULL	42 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	To assess the significance of radiographic signs of sclerosis of the third carpal bone ( C3 ) in young Standardbred trotters in relation to performance , lameness and bone turnover both carpi in 14 Standardbred trotters were radiographically and scintigraphically examined 6 times , from the beginning of speed training until the beginning of racing , between the mean ages of 20 and 42 months .
	manualset3
216255	1	419944	7	NULL	NULL	0	NULL	Sensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitivity for cancer was also high , but false negative rate was lower with TV than TA .
	manualset3
216256	2	419944	7	NULL	NULL	0	NULL	 cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitivity for cancer was also high , but false negative rate was lower with TV than TA .
	manualset3
216257	3	419944	7	NULL	NULL	0	NULL	false negative rate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitivity for cancer was also high , but false negative rate was lower with TV than TA .
	manualset3
216258	4	419944	7	NULL	NULL	0	NULL	TV 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitivity for cancer was also high , but false negative rate was lower with TV than TA .
	manualset3
216259	5	419944	7	NULL	NULL	0	NULL	TA	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitivity for cancer was also high , but false negative rate was lower with TV than TA .
	manualset3
216260	1	419945	7	NULL	NULL	NULL	NULL	tablet erosion	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The tablet erosion was studied in a modified USP II apparatus at different agitation intensities and ionic strengths according to 2 ( 2 ) factorial design .
	manualset3
216261	2	419945	7	NULL	NULL	0	NULL	modified USP II apparatus	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The tablet erosion was studied in a modified USP II apparatus at different agitation intensities and ionic strengths according to 2 ( 2 ) factorial design .
	manualset3
216262	3	419945	7	NULL	NULL	0	NULL	agitation intensities	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The tablet erosion was studied in a modified USP II apparatus at different agitation intensities and ionic strengths according to 2 ( 2 ) factorial design .
	manualset3
216263	4	419945	7	NULL	NULL	0	NULL	ionic strengths	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The tablet erosion was studied in a modified USP II apparatus at different agitation intensities and ionic strengths according to 2 ( 2 ) factorial design .
	manualset3
216264	5	419945	7	NULL	NULL	0	NULL	2 ( 2 ) factorial design	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The tablet erosion was studied in a modified USP II apparatus at different agitation intensities and ionic strengths according to 2 ( 2 ) factorial design .
	manualset3
216265	1	419946	7	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the growth of KUCaP in male mice was androgen dependent , bicalutamide aberrantly promoted the growth and prostate-specific antigen production of KUCaP .
	manualset3
216266	2	419946	7	NULL	NULL	0	NULL	KUCaP	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the growth of KUCaP in male mice was androgen dependent , bicalutamide aberrantly promoted the growth and prostate-specific antigen production of KUCaP .
	manualset3
216267	3	419946	7	NULL	NULL	0	NULL	male mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the growth of KUCaP in male mice was androgen dependent , bicalutamide aberrantly promoted the growth and prostate-specific antigen production of KUCaP .
	manualset3
216268	4	419946	7	NULL	NULL	0	NULL	bicalutamide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the growth of KUCaP in male mice was androgen dependent , bicalutamide aberrantly promoted the growth and prostate-specific antigen production of KUCaP .
	manualset3
216269	5	419946	7	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the growth of KUCaP in male mice was androgen dependent , bicalutamide aberrantly promoted the growth and prostate-specific antigen production of KUCaP .
	manualset3
216270	6	419946	7	NULL	NULL	0	NULL	prostate-specific antigen production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the growth of KUCaP in male mice was androgen dependent , bicalutamide aberrantly promoted the growth and prostate-specific antigen production of KUCaP .
	manualset3
216271	7	419946	7	NULL	NULL	0	NULL	KUCaP 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the growth of KUCaP in male mice was androgen dependent , bicalutamide aberrantly promoted the growth and prostate-specific antigen production of KUCaP .
	manualset3
216272	1	419947	7	NULL	NULL	0	NULL	Compartment syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Compartment syndrome was diagnosed in five patients on the basis of clinical findings , and the diagnosis was confirmed when peak compartment pressures of more than the critical threshold ( within twenty millimeters of mercury ( 2.67 kilopascals ) of the diastolic blood pressure ) were recorded .
	manualset3
216273	2	419947	7	NULL	NULL	0	NULL	five patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Compartment syndrome was diagnosed in five patients on the basis of clinical findings , and the diagnosis was confirmed when peak compartment pressures of more than the critical threshold ( within twenty millimeters of mercury ( 2.67 kilopascals ) of the diastolic blood pressure ) were recorded .
	manualset3
216274	3	419947	7	NULL	NULL	0	NULL	 basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compartment syndrome was diagnosed in five patients on the basis of clinical findings , and the diagnosis was confirmed when peak compartment pressures of more than the critical threshold ( within twenty millimeters of mercury ( 2.67 kilopascals ) of the diastolic blood pressure ) were recorded .
	manualset3
216275	4	419947	7	NULL	NULL	0	NULL	clinical findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Compartment syndrome was diagnosed in five patients on the basis of clinical findings , and the diagnosis was confirmed when peak compartment pressures of more than the critical threshold ( within twenty millimeters of mercury ( 2.67 kilopascals ) of the diastolic blood pressure ) were recorded .
	manualset3
216276	5	419947	7	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Compartment syndrome was diagnosed in five patients on the basis of clinical findings , and the diagnosis was confirmed when peak compartment pressures of more than the critical threshold ( within twenty millimeters of mercury ( 2.67 kilopascals ) of the diastolic blood pressure ) were recorded .
	manualset3
216277	6	419947	7	NULL	NULL	0	NULL	peak compartment pressures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compartment syndrome was diagnosed in five patients on the basis of clinical findings , and the diagnosis was confirmed when peak compartment pressures of more than the critical threshold ( within twenty millimeters of mercury ( 2.67 kilopascals ) of the diastolic blood pressure ) were recorded .
	manualset3
216278	7	419947	7	NULL	NULL	0	NULL	critical threshold 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compartment syndrome was diagnosed in five patients on the basis of clinical findings , and the diagnosis was confirmed when peak compartment pressures of more than the critical threshold ( within twenty millimeters of mercury ( 2.67 kilopascals ) of the diastolic blood pressure ) were recorded .
	manualset3
216279	8	419947	7	NULL	NULL	0	NULL	twenty millimeters 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Compartment syndrome was diagnosed in five patients on the basis of clinical findings , and the diagnosis was confirmed when peak compartment pressures of more than the critical threshold ( within twenty millimeters of mercury ( 2.67 kilopascals ) of the diastolic blood pressure ) were recorded .
	manualset3
216280	9	419947	7	NULL	NULL	0	NULL	mercury	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compartment syndrome was diagnosed in five patients on the basis of clinical findings , and the diagnosis was confirmed when peak compartment pressures of more than the critical threshold ( within twenty millimeters of mercury ( 2.67 kilopascals ) of the diastolic blood pressure ) were recorded .
	manualset3
216281	10	419947	7	NULL	NULL	0	NULL	2.67 kilopascals 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compartment syndrome was diagnosed in five patients on the basis of clinical findings , and the diagnosis was confirmed when peak compartment pressures of more than the critical threshold ( within twenty millimeters of mercury ( 2.67 kilopascals ) of the diastolic blood pressure ) were recorded .
	manualset3
216282	11	419947	7	NULL	NULL	0	NULL	diastolic blood pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Compartment syndrome was diagnosed in five patients on the basis of clinical findings , and the diagnosis was confirmed when peak compartment pressures of more than the critical threshold ( within twenty millimeters of mercury ( 2.67 kilopascals ) of the diastolic blood pressure ) were recorded .
	manualset3
216283	1	419948	7	NULL	NULL	0	NULL	RA injections	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For RA injections the relationship between delta MTT and CO-1 was linear in all experiments , with an average correlation coefficient of 0.97 + / - 0.01 ( SE ) , indicating that the VODev was constant over a threefold increase in CO. .
	manualset3
216284	2	419948	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	For RA injections the relationship between delta MTT and CO-1 was linear in all experiments , with an average correlation coefficient of 0.97 + / - 0.01 ( SE ) , indicating that the VODev was constant over a threefold increase in CO. .
	manualset3
216285	3	419948	7	NULL	NULL	0	NULL	delta MTT	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For RA injections the relationship between delta MTT and CO-1 was linear in all experiments , with an average correlation coefficient of 0.97 + / - 0.01 ( SE ) , indicating that the VODev was constant over a threefold increase in CO. .
	manualset3
216286	4	419948	7	NULL	NULL	0	NULL	CO-1	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For RA injections the relationship between delta MTT and CO-1 was linear in all experiments , with an average correlation coefficient of 0.97 + / - 0.01 ( SE ) , indicating that the VODev was constant over a threefold increase in CO. .
	manualset3
216287	5	419948	7	NULL	NULL	0	NULL	experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For RA injections the relationship between delta MTT and CO-1 was linear in all experiments , with an average correlation coefficient of 0.97 + / - 0.01 ( SE ) , indicating that the VODev was constant over a threefold increase in CO. .
	manualset3
216288	6	419948	7	NULL	NULL	0	NULL	average correlation coefficient	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For RA injections the relationship between delta MTT and CO-1 was linear in all experiments , with an average correlation coefficient of 0.97 + / - 0.01 ( SE ) , indicating that the VODev was constant over a threefold increase in CO. .
	manualset3
216289	7	419948	7	NULL	NULL	0	NULL	0.97 + / - 0.01 ( SE ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For RA injections the relationship between delta MTT and CO-1 was linear in all experiments , with an average correlation coefficient of 0.97 + / - 0.01 ( SE ) , indicating that the VODev was constant over a threefold increase in CO. .
	manualset3
216290	8	419948	7	NULL	NULL	0	NULL	VODev	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For RA injections the relationship between delta MTT and CO-1 was linear in all experiments , with an average correlation coefficient of 0.97 + / - 0.01 ( SE ) , indicating that the VODev was constant over a threefold increase in CO. .
	manualset3
216291	9	419948	7	NULL	NULL	0	NULL	threefold increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For RA injections the relationship between delta MTT and CO-1 was linear in all experiments , with an average correlation coefficient of 0.97 + / - 0.01 ( SE ) , indicating that the VODev was constant over a threefold increase in CO. .
	manualset3
216292	10	419948	7	NULL	NULL	0	NULL	CO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For RA injections the relationship between delta MTT and CO-1 was linear in all experiments , with an average correlation coefficient of 0.97 + / - 0.01 ( SE ) , indicating that the VODev was constant over a threefold increase in CO. .
	manualset3
216293	1	419949	7	NULL	NULL	0	NULL	Intra-lymphatic injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intra-lymphatic injection of cyclophosphamide .
	manualset3
216294	2	419949	7	NULL	NULL	NULL	NULL	cyclophosphamide	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Intra-lymphatic injection of cyclophosphamide .
	manualset3
216295	1	419950	7	NULL	NULL	0	NULL	Intracerebroventricular administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracerebroventricular administration of dopamine also induced a significant reduction of NTLI concentration and Bmax of NT receptor with no change in Kd .
	manualset3
216296	2	419950	7	NULL	NULL	0	NULL	dopamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracerebroventricular administration of dopamine also induced a significant reduction of NTLI concentration and Bmax of NT receptor with no change in Kd .
	manualset3
216297	3	419950	7	NULL	NULL	0	NULL	significant reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracerebroventricular administration of dopamine also induced a significant reduction of NTLI concentration and Bmax of NT receptor with no change in Kd .
	manualset3
216298	4	419950	7	NULL	NULL	0	NULL	NTLI concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracerebroventricular administration of dopamine also induced a significant reduction of NTLI concentration and Bmax of NT receptor with no change in Kd .
	manualset3
216299	5	419950	7	NULL	NULL	0	NULL	Bmax	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracerebroventricular administration of dopamine also induced a significant reduction of NTLI concentration and Bmax of NT receptor with no change in Kd .
	manualset3
216300	6	419950	7	NULL	NULL	0	NULL	NT receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracerebroventricular administration of dopamine also induced a significant reduction of NTLI concentration and Bmax of NT receptor with no change in Kd .
	manualset3
216301	7	419950	7	NULL	NULL	0	NULL	Kd	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracerebroventricular administration of dopamine also induced a significant reduction of NTLI concentration and Bmax of NT receptor with no change in Kd .
	manualset3
216302	1	419951	7	NULL	NULL	0	NULL	Interactions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions of 57Co , 85Sr and 137Cs with peat under acidic precipitation conditions .
	manualset3
216303	2	419951	7	NULL	NULL	0	NULL	57Co	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions of 57Co , 85Sr and 137Cs with peat under acidic precipitation conditions .
	manualset3
216304	3	419951	7	NULL	NULL	0	NULL	85Sr	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions of 57Co , 85Sr and 137Cs with peat under acidic precipitation conditions .
	manualset3
216305	4	419951	7	NULL	NULL	0	NULL	137Cs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions of 57Co , 85Sr and 137Cs with peat under acidic precipitation conditions .
	manualset3
216306	5	419951	7	NULL	NULL	0	NULL	peat	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions of 57Co , 85Sr and 137Cs with peat under acidic precipitation conditions .
	manualset3
216307	6	419951	7	NULL	NULL	NULL	NULL	acidic precipitation conditions	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Interactions of 57Co , 85Sr and 137Cs with peat under acidic precipitation conditions .
	manualset3
216308	1	419952	7	NULL	NULL	0	NULL	Speciation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Speciation in solution of the systems Cu/HL and Cu/L ( 1 ) have been determined by means of potentiometry and spectrophotometry as well as for the Cu/L ( 1 ) / A ( HA = glycine ) system in order to determine species present at physiological pH. .
	manualset3
216309	2	419952	7	NULL	NULL	0	NULL	solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Speciation in solution of the systems Cu/HL and Cu/L ( 1 ) have been determined by means of potentiometry and spectrophotometry as well as for the Cu/L ( 1 ) / A ( HA = glycine ) system in order to determine species present at physiological pH. .
	manualset3
216310	3	419952	7	NULL	NULL	0	NULL	systems	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Speciation in solution of the systems Cu/HL and Cu/L ( 1 ) have been determined by means of potentiometry and spectrophotometry as well as for the Cu/L ( 1 ) / A ( HA = glycine ) system in order to determine species present at physiological pH. .
	manualset3
216311	4	419952	7	NULL	NULL	0	NULL	Cu/HL	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Speciation in solution of the systems Cu/HL and Cu/L ( 1 ) have been determined by means of potentiometry and spectrophotometry as well as for the Cu/L ( 1 ) / A ( HA = glycine ) system in order to determine species present at physiological pH. .
	manualset3
216312	5	419952	7	NULL	NULL	0	NULL	Cu/L ( 1 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Speciation in solution of the systems Cu/HL and Cu/L ( 1 ) have been determined by means of potentiometry and spectrophotometry as well as for the Cu/L ( 1 ) / A ( HA = glycine ) system in order to determine species present at physiological pH. .
	manualset3
216313	6	419952	7	NULL	NULL	0	NULL	potentiometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Speciation in solution of the systems Cu/HL and Cu/L ( 1 ) have been determined by means of potentiometry and spectrophotometry as well as for the Cu/L ( 1 ) / A ( HA = glycine ) system in order to determine species present at physiological pH. .
	manualset3
216314	7	419952	7	NULL	NULL	0	NULL	spectrophotometry 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Speciation in solution of the systems Cu/HL and Cu/L ( 1 ) have been determined by means of potentiometry and spectrophotometry as well as for the Cu/L ( 1 ) / A ( HA = glycine ) system in order to determine species present at physiological pH. .
	manualset3
216315	8	419952	7	NULL	NULL	NULL	NULL	Cu/L ( 1 ) / A system	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Speciation in solution of the systems Cu/HL and Cu/L ( 1 ) have been determined by means of potentiometry and spectrophotometry as well as for the Cu/L ( 1 ) / A ( HA = glycine ) system in order to determine species present at physiological pH. .
	manualset3
216316	9	419952	7	NULL	NULL	0	NULL	HA = glycine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Speciation in solution of the systems Cu/HL and Cu/L ( 1 ) have been determined by means of potentiometry and spectrophotometry as well as for the Cu/L ( 1 ) / A ( HA = glycine ) system in order to determine species present at physiological pH. .
	manualset3
216317	10	419952	7	NULL	NULL	0	NULL	species 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Speciation in solution of the systems Cu/HL and Cu/L ( 1 ) have been determined by means of potentiometry and spectrophotometry as well as for the Cu/L ( 1 ) / A ( HA = glycine ) system in order to determine species present at physiological pH. .
	manualset3
216318	11	419952	7	NULL	NULL	0	NULL	physiological pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Speciation in solution of the systems Cu/HL and Cu/L ( 1 ) have been determined by means of potentiometry and spectrophotometry as well as for the Cu/L ( 1 ) / A ( HA = glycine ) system in order to determine species present at physiological pH. .
	manualset3
216319	1	419953	7	NULL	NULL	0	NULL	high titer vaccines	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the high titer vaccines are more immunogenic in young infants than standard vaccines , long term safety must be assured before these vaccines can be put into widespread use .
	manualset3
216320	2	419953	7	NULL	NULL	0	NULL	young infants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the high titer vaccines are more immunogenic in young infants than standard vaccines , long term safety must be assured before these vaccines can be put into widespread use .
	manualset3
216321	3	419953	7	NULL	NULL	0	NULL	standard vaccines	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the high titer vaccines are more immunogenic in young infants than standard vaccines , long term safety must be assured before these vaccines can be put into widespread use .
	manualset3
216322	4	419953	7	NULL	NULL	0	NULL	long term safety	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the high titer vaccines are more immunogenic in young infants than standard vaccines , long term safety must be assured before these vaccines can be put into widespread use .
	manualset3
216323	5	419953	7	NULL	NULL	0	NULL	vaccines	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the high titer vaccines are more immunogenic in young infants than standard vaccines , long term safety must be assured before these vaccines can be put into widespread use .
	manualset3
216324	1	419954	7	NULL	NULL	0	NULL	follicular fluid	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Presumably , the follicular fluid and endometrium samples contain active factors which function as radical scavengers .
	manualset3
216325	2	419954	7	NULL	NULL	0	NULL	endometrium samples 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Presumably , the follicular fluid and endometrium samples contain active factors which function as radical scavengers .
	manualset3
216326	3	419954	7	NULL	NULL	0	NULL	active factors	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Presumably , the follicular fluid and endometrium samples contain active factors which function as radical scavengers .
	manualset3
216327	4	419954	7	NULL	NULL	0	NULL	radical scavengers	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Presumably , the follicular fluid and endometrium samples contain active factors which function as radical scavengers .
	manualset3
216328	1	419955	7	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We were looking for a possible risk of infection associated with animal contacts .
	manualset3
216329	2	419955	7	NULL	NULL	0	NULL	 infection	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We were looking for a possible risk of infection associated with animal contacts .
	manualset3
216330	3	419955	7	NULL	NULL	0	NULL	animal contacts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We were looking for a possible risk of infection associated with animal contacts .
	manualset3
216331	1	419956	7	NULL	NULL	0	NULL	Chronic neuropathic pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic neuropathic pain in spinal cord injury : efficiency of deep brain and motor cortex stimulation therapies for neuropathic pain in spinal cord injury patients .
	manualset3
216332	2	419956	7	NULL	NULL	0	NULL	 spinal cord injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic neuropathic pain in spinal cord injury : efficiency of deep brain and motor cortex stimulation therapies for neuropathic pain in spinal cord injury patients .
	manualset3
216333	3	419956	7	NULL	NULL	0	NULL	deep brain stimulation therapies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic neuropathic pain in spinal cord injury : efficiency of deep brain and motor cortex stimulation therapies for neuropathic pain in spinal cord injury patients .
	manualset3
216334	4	419956	7	NULL	NULL	0	NULL	motor cortex stimulation therapies 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic neuropathic pain in spinal cord injury : efficiency of deep brain and motor cortex stimulation therapies for neuropathic pain in spinal cord injury patients .
	manualset3
216335	5	419956	7	NULL	NULL	0	NULL	neuropathic pain 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic neuropathic pain in spinal cord injury : efficiency of deep brain and motor cortex stimulation therapies for neuropathic pain in spinal cord injury patients .
	manualset3
216336	6	419956	7	NULL	NULL	0	NULL	spinal cord injury patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic neuropathic pain in spinal cord injury : efficiency of deep brain and motor cortex stimulation therapies for neuropathic pain in spinal cord injury patients .
	manualset3
216337	1	419957	7	NULL	NULL	0	NULL	incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the incidence of anastomotic leakage is reportedly high , the authors observed anastomotic leakage in only one of eight patients .
	manualset3
216338	2	419957	7	NULL	NULL	0	NULL	anastomotic leakage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the incidence of anastomotic leakage is reportedly high , the authors observed anastomotic leakage in only one of eight patients .
	manualset3
216339	3	419957	7	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the incidence of anastomotic leakage is reportedly high , the authors observed anastomotic leakage in only one of eight patients .
	manualset3
216340	4	419957	7	NULL	NULL	0	NULL	anastomotic leakage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the incidence of anastomotic leakage is reportedly high , the authors observed anastomotic leakage in only one of eight patients .
	manualset3
216341	5	419957	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the incidence of anastomotic leakage is reportedly high , the authors observed anastomotic leakage in only one of eight patients .
	manualset3
216342	6	419957	7	NULL	NULL	0	NULL	eight patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the incidence of anastomotic leakage is reportedly high , the authors observed anastomotic leakage in only one of eight patients .
	manualset3
216343	1	419958	7	NULL	NULL	0	NULL	Simultaneous stereoselective high-performance liquid chromatographic determination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous stereoselective high-performance liquid chromatographic determination of 10-hydroxycarbazepine and its metabolite carbamazepine-10 , 11 - trans-dihydrodiol in human urine .
	manualset3
216344	2	419958	7	NULL	NULL	0	NULL	10-hydroxycarbazepine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous stereoselective high-performance liquid chromatographic determination of 10-hydroxycarbazepine and its metabolite carbamazepine-10 , 11 - trans-dihydrodiol in human urine .
	manualset3
216345	3	419958	7	NULL	NULL	0	NULL	metabolite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous stereoselective high-performance liquid chromatographic determination of 10-hydroxycarbazepine and its metabolite carbamazepine-10 , 11 - trans-dihydrodiol in human urine .
	manualset3
216346	4	419958	7	NULL	NULL	0	NULL	carbamazepine-10 , 11 - trans-dihydrodiol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous stereoselective high-performance liquid chromatographic determination of 10-hydroxycarbazepine and its metabolite carbamazepine-10 , 11 - trans-dihydrodiol in human urine .
	manualset3
216347	5	419958	7	NULL	NULL	0	NULL	human urine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous stereoselective high-performance liquid chromatographic determination of 10-hydroxycarbazepine and its metabolite carbamazepine-10 , 11 - trans-dihydrodiol in human urine .
	manualset3
216348	1	419959	7	NULL	NULL	0	NULL	dense meshwork	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	This may be associated with a dense meshwork of membrane junctions between neighboring microvilli as revealed by electron microscope image analysis .
	manualset3
216349	2	419959	7	NULL	NULL	0	NULL	membrane junctions	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	This may be associated with a dense meshwork of membrane junctions between neighboring microvilli as revealed by electron microscope image analysis .
	manualset3
216350	3	419959	7	NULL	NULL	0	NULL	neighboring microvilli	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This may be associated with a dense meshwork of membrane junctions between neighboring microvilli as revealed by electron microscope image analysis .
	manualset3
216351	4	419959	7	NULL	NULL	0	NULL	electron microscope image analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This may be associated with a dense meshwork of membrane junctions between neighboring microvilli as revealed by electron microscope image analysis .
	manualset3
216352	1	419960	7	NULL	NULL	0	NULL	HEXA gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The HEXA gene for Tay-Sachs was cloned at the National Institutes of Health , and the gene was patented but has not been licensed .
	manualset3
216353	2	419960	7	NULL	NULL	0	NULL	Tay-Sachs	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The HEXA gene for Tay-Sachs was cloned at the National Institutes of Health , and the gene was patented but has not been licensed .
	manualset3
216354	3	419960	7	NULL	NULL	0	NULL	National Institutes of Health	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The HEXA gene for Tay-Sachs was cloned at the National Institutes of Health , and the gene was patented but has not been licensed .
	manualset3
216355	4	419960	7	NULL	NULL	0	NULL	gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The HEXA gene for Tay-Sachs was cloned at the National Institutes of Health , and the gene was patented but has not been licensed .
	manualset3
216356	1	419961	7	NULL	NULL	0	NULL	 addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of vincristine to the program 7 + 3 failed to make remission more frequent and recurrence-free survival longer .
	manualset3
216357	2	419961	7	NULL	NULL	0	NULL	vincristine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of vincristine to the program 7 + 3 failed to make remission more frequent and recurrence-free survival longer .
	manualset3
216358	3	419961	7	NULL	NULL	0	NULL	 program 7 + 3	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of vincristine to the program 7 + 3 failed to make remission more frequent and recurrence-free survival longer .
	manualset3
216359	4	419961	7	NULL	NULL	0	NULL	remission	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of vincristine to the program 7 + 3 failed to make remission more frequent and recurrence-free survival longer .
	manualset3
216360	5	419961	7	NULL	NULL	0	NULL	recurrence-free survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of vincristine to the program 7 + 3 failed to make remission more frequent and recurrence-free survival longer .
	manualset3
216361	1	419962	7	NULL	NULL	0	NULL	age	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Their age mean + / - SD 38.2 + / - 11.1 years , ad had completed 3.8 + / - 2.2 years after transplantation .
	manualset3
216362	2	419962	7	NULL	NULL	0	NULL	+ / - SD 38.2 + / - 11.1 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Their age mean + / - SD 38.2 + / - 11.1 years , ad had completed 3.8 + / - 2.2 years after transplantation .
	manualset3
216363	3	419962	7	NULL	NULL	0	NULL	3.8 + / - 2.2 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Their age mean + / - SD 38.2 + / - 11.1 years , ad had completed 3.8 + / - 2.2 years after transplantation .
	manualset3
216364	4	419962	7	NULL	NULL	0	NULL	transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Their age mean + / - SD 38.2 + / - 11.1 years , ad had completed 3.8 + / - 2.2 years after transplantation .
	manualset3
216365	1	419963	7	NULL	NULL	0	NULL	electrode E2 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrode E2 was also used to determine concentrations of thiocyanate in biological samples .
	manualset3
216366	2	419963	7	NULL	NULL	0	NULL	concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrode E2 was also used to determine concentrations of thiocyanate in biological samples .
	manualset3
216367	3	419963	7	NULL	NULL	0	NULL	thiocyanate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrode E2 was also used to determine concentrations of thiocyanate in biological samples .
	manualset3
216368	4	419963	7	NULL	NULL	0	NULL	biological samples 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The electrode E2 was also used to determine concentrations of thiocyanate in biological samples .
	manualset3
216369	1	419964	7	NULL	NULL	0	NULL	 induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of the HO-1 gene expression by OA was transcriptional as determined by studies with actinomycin D , nuclear run-off assay , and measurement of the half-life of HO-1 mRNA .
	manualset3
216370	2	419964	7	NULL	NULL	0	NULL	HO-1 gene expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of the HO-1 gene expression by OA was transcriptional as determined by studies with actinomycin D , nuclear run-off assay , and measurement of the half-life of HO-1 mRNA .
	manualset3
216371	3	419964	7	NULL	NULL	0	NULL	 OA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of the HO-1 gene expression by OA was transcriptional as determined by studies with actinomycin D , nuclear run-off assay , and measurement of the half-life of HO-1 mRNA .
	manualset3
216372	4	419964	7	NULL	NULL	0	NULL	actinomycin D	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of the HO-1 gene expression by OA was transcriptional as determined by studies with actinomycin D , nuclear run-off assay , and measurement of the half-life of HO-1 mRNA .
	manualset3
216373	5	419964	7	NULL	NULL	0	NULL	nuclear run-off assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of the HO-1 gene expression by OA was transcriptional as determined by studies with actinomycin D , nuclear run-off assay , and measurement of the half-life of HO-1 mRNA .
	manualset3
216374	6	419964	7	NULL	NULL	NULL	NULL	measurement	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The induction of the HO-1 gene expression by OA was transcriptional as determined by studies with actinomycin D , nuclear run-off assay , and measurement of the half-life of HO-1 mRNA .
	manualset3
216375	7	419964	7	NULL	NULL	0	NULL	half-life 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of the HO-1 gene expression by OA was transcriptional as determined by studies with actinomycin D , nuclear run-off assay , and measurement of the half-life of HO-1 mRNA .
	manualset3
216376	8	419964	7	NULL	NULL	0	NULL	HO-1 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of the HO-1 gene expression by OA was transcriptional as determined by studies with actinomycin D , nuclear run-off assay , and measurement of the half-life of HO-1 mRNA .
	manualset3
217439	9	419964	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The induction of the HO-1 gene expression by OA was transcriptional as determined by studies with actinomycin D , nuclear run-off assay , and measurement of the half-life of HO-1 mRNA .
	manualset3
216377	1	419965	7	NULL	NULL	0	NULL	ligand-induced RET signaling pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the ligand-induced RET signaling pathway has been well described , little is known about the regulation of RET surface expression , which is integral to the cell ability to control the response to ligand stimuli .
	manualset3
216378	2	419965	7	NULL	NULL	0	NULL	regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the ligand-induced RET signaling pathway has been well described , little is known about the regulation of RET surface expression , which is integral to the cell ability to control the response to ligand stimuli .
	manualset3
216379	3	419965	7	NULL	NULL	0	NULL	RET surface expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the ligand-induced RET signaling pathway has been well described , little is known about the regulation of RET surface expression , which is integral to the cell ability to control the response to ligand stimuli .
	manualset3
216380	4	419965	7	NULL	NULL	0	NULL	cell ability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the ligand-induced RET signaling pathway has been well described , little is known about the regulation of RET surface expression , which is integral to the cell ability to control the response to ligand stimuli .
	manualset3
216381	5	419965	7	NULL	NULL	0	NULL	ligand stimuli 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the ligand-induced RET signaling pathway has been well described , little is known about the regulation of RET surface expression , which is integral to the cell ability to control the response to ligand stimuli .
	manualset3
216382	6	419965	7	NULL	NULL	0	NULL	response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the ligand-induced RET signaling pathway has been well described , little is known about the regulation of RET surface expression , which is integral to the cell ability to control the response to ligand stimuli .
	manualset3
216383	1	419966	7	NULL	NULL	0	NULL	Tesofensine ( TE ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Tesofensine ( TE ) , an inhibitor of monoamine presynaptic reuptake , has produced twice the weight loss seen with currently marketed drugs .
	manualset3
216384	2	419966	7	NULL	NULL	0	NULL	inhibitor 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Tesofensine ( TE ) , an inhibitor of monoamine presynaptic reuptake , has produced twice the weight loss seen with currently marketed drugs .
	manualset3
216385	3	419966	7	NULL	NULL	0	NULL	monoamine presynaptic reuptake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Tesofensine ( TE ) , an inhibitor of monoamine presynaptic reuptake , has produced twice the weight loss seen with currently marketed drugs .
	manualset3
216386	4	419966	7	NULL	NULL	0	NULL	 weight loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Tesofensine ( TE ) , an inhibitor of monoamine presynaptic reuptake , has produced twice the weight loss seen with currently marketed drugs .
	manualset3
216387	5	419966	7	NULL	NULL	0	NULL	drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Tesofensine ( TE ) , an inhibitor of monoamine presynaptic reuptake , has produced twice the weight loss seen with currently marketed drugs .
	manualset3
216388	1	419967	7	NULL	NULL	0	NULL	integrating volume sets	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	By integrating volume sets of flow images , two-dimensional images of blood vessels are obtained .
	manualset3
216389	2	419967	7	NULL	NULL	0	NULL	flow images	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	By integrating volume sets of flow images , two-dimensional images of blood vessels are obtained .
	manualset3
216390	3	419967	7	NULL	NULL	0	NULL	 two-dimensional images	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	By integrating volume sets of flow images , two-dimensional images of blood vessels are obtained .
	manualset3
216391	4	419967	7	NULL	NULL	0	NULL	blood vessels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	By integrating volume sets of flow images , two-dimensional images of blood vessels are obtained .
	manualset3
216392	1	419968	7	NULL	NULL	0	NULL	carotenoids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These carotenoids produced by the recombinant P. pastoris clones were qualitatively and quantitatively analyzed by high-resolution liquid chromatography , coupled to photodiode array detector .
	manualset3
216393	2	419968	7	NULL	NULL	0	NULL	recombinant P. pastoris clones	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These carotenoids produced by the recombinant P. pastoris clones were qualitatively and quantitatively analyzed by high-resolution liquid chromatography , coupled to photodiode array detector .
	manualset3
216394	3	419968	7	NULL	NULL	0	NULL	high-resolution liquid chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These carotenoids produced by the recombinant P. pastoris clones were qualitatively and quantitatively analyzed by high-resolution liquid chromatography , coupled to photodiode array detector .
	manualset3
216395	4	419968	7	NULL	NULL	0	NULL	photodiode array detector .	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	These carotenoids produced by the recombinant P. pastoris clones were qualitatively and quantitatively analyzed by high-resolution liquid chromatography , coupled to photodiode array detector .
	manualset3
216396	1	419969	7	NULL	NULL	0	NULL	SiRNA-mediated knockdown analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	SiRNA-mediated knockdown and reporter gene analyses identified two transcription factors , homeodomain protein MSX1 and bZIP protein XBP1 , directly regulating ZHX2 expression .
	manualset3
216397	2	419969	7	NULL	NULL	0	NULL	reporter gene analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	SiRNA-mediated knockdown and reporter gene analyses identified two transcription factors , homeodomain protein MSX1 and bZIP protein XBP1 , directly regulating ZHX2 expression .
	manualset3
216398	3	419969	7	NULL	NULL	0	NULL	two transcription factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	SiRNA-mediated knockdown and reporter gene analyses identified two transcription factors , homeodomain protein MSX1 and bZIP protein XBP1 , directly regulating ZHX2 expression .
	manualset3
216399	4	419969	7	NULL	NULL	0	NULL	homeodomain protein MSX1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	SiRNA-mediated knockdown and reporter gene analyses identified two transcription factors , homeodomain protein MSX1 and bZIP protein XBP1 , directly regulating ZHX2 expression .
	manualset3
216400	5	419969	7	NULL	NULL	0	NULL	bZIP protein XBP1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	SiRNA-mediated knockdown and reporter gene analyses identified two transcription factors , homeodomain protein MSX1 and bZIP protein XBP1 , directly regulating ZHX2 expression .
	manualset3
216401	6	419969	7	NULL	NULL	NULL	NULL	ZHX2 expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	SiRNA-mediated knockdown and reporter gene analyses identified two transcription factors , homeodomain protein MSX1 and bZIP protein XBP1 , directly regulating ZHX2 expression .
	manualset3
216402	1	419970	7	NULL	NULL	0	NULL	Rehabilitation laws 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Rehabilitation laws and hospitals ) .
	manualset3
216403	2	419970	7	NULL	NULL	0	NULL	hospitals 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( Rehabilitation laws and hospitals ) .
	manualset3
216404	1	419971	7	NULL	NULL	0	NULL	 lung	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the lung normally maintains its alveoli dry , during ARDS increased permeability of small pulmonary vessels results in primary pulmonary edema , in contrast to edema from increased vascular pressure .
	manualset3
216405	2	419971	7	NULL	NULL	0	NULL	alveoli	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the lung normally maintains its alveoli dry , during ARDS increased permeability of small pulmonary vessels results in primary pulmonary edema , in contrast to edema from increased vascular pressure .
	manualset3
216406	3	419971	7	NULL	NULL	0	NULL	ARDS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the lung normally maintains its alveoli dry , during ARDS increased permeability of small pulmonary vessels results in primary pulmonary edema , in contrast to edema from increased vascular pressure .
	manualset3
216407	4	419971	7	NULL	NULL	0	NULL	permeability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the lung normally maintains its alveoli dry , during ARDS increased permeability of small pulmonary vessels results in primary pulmonary edema , in contrast to edema from increased vascular pressure .
	manualset3
216408	5	419971	7	NULL	NULL	0	NULL	small pulmonary vessels 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the lung normally maintains its alveoli dry , during ARDS increased permeability of small pulmonary vessels results in primary pulmonary edema , in contrast to edema from increased vascular pressure .
	manualset3
216409	6	419971	7	NULL	NULL	0	NULL	primary pulmonary edema	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the lung normally maintains its alveoli dry , during ARDS increased permeability of small pulmonary vessels results in primary pulmonary edema , in contrast to edema from increased vascular pressure .
	manualset3
216410	7	419971	7	NULL	NULL	0	NULL	edema 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the lung normally maintains its alveoli dry , during ARDS increased permeability of small pulmonary vessels results in primary pulmonary edema , in contrast to edema from increased vascular pressure .
	manualset3
216411	8	419971	7	NULL	NULL	0	NULL	vascular pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the lung normally maintains its alveoli dry , during ARDS increased permeability of small pulmonary vessels results in primary pulmonary edema , in contrast to edema from increased vascular pressure .
	manualset3
216412	1	419972	7	NULL	NULL	0	NULL	Haematological parameters 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Haematological parameters , blood chemistry and serum levels of non specific IgE were also measured .
	manualset3
216413	2	419972	7	NULL	NULL	0	NULL	 blood chemistry	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Haematological parameters , blood chemistry and serum levels of non specific IgE were also measured .
	manualset3
216414	3	419972	7	NULL	NULL	0	NULL	serum levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Haematological parameters , blood chemistry and serum levels of non specific IgE were also measured .
	manualset3
216415	4	419972	7	NULL	NULL	0	NULL	non specific IgE	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Haematological parameters , blood chemistry and serum levels of non specific IgE were also measured .
	manualset3
216416	1	419973	7	NULL	NULL	0	NULL	Differentiation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Differentiation of oxidative and nonglucolytic Gram-negative bacteria .
	manualset3
216417	2	419973	7	NULL	NULL	0	NULL	oxidative Gram-negative bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Differentiation of oxidative and nonglucolytic Gram-negative bacteria .
	manualset3
216418	3	419973	7	NULL	NULL	0	NULL	nonglucolytic Gram-negative bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Differentiation of oxidative and nonglucolytic Gram-negative bacteria .
	manualset3
216419	1	419974	7	NULL	NULL	0	NULL	Pulmonary valvotomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary valvotomy : an alternative method .
	manualset3
216420	2	419974	7	NULL	NULL	NULL	NULL	alternative method	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pulmonary valvotomy : an alternative method .
	manualset3
216421	1	419975	7	NULL	NULL	NULL	NULL	inhomogeneous distribution 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The inhomogeneous distribution of MS may represent an important clue about the cause of the disease .
	manualset3
216422	2	419975	7	NULL	NULL	0	NULL	MS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhomogeneous distribution of MS may represent an important clue about the cause of the disease .
	manualset3
216423	3	419975	7	NULL	NULL	0	NULL	clue	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhomogeneous distribution of MS may represent an important clue about the cause of the disease .
	manualset3
216424	4	419975	7	NULL	NULL	0	NULL	cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhomogeneous distribution of MS may represent an important clue about the cause of the disease .
	manualset3
216425	5	419975	7	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhomogeneous distribution of MS may represent an important clue about the cause of the disease .
	manualset3
216426	1	419976	7	NULL	NULL	0	NULL	mouse hepatocellular carcinoma cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The mouse hepatocellular carcinoma cell line Hepa 1-6 was used as a model in this study .
	manualset3
216427	2	419976	7	NULL	NULL	0	NULL	Hepa 1-6	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The mouse hepatocellular carcinoma cell line Hepa 1-6 was used as a model in this study .
	manualset3
216428	3	419976	7	NULL	NULL	0	NULL	model 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The mouse hepatocellular carcinoma cell line Hepa 1-6 was used as a model in this study .
	manualset3
216429	4	419976	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The mouse hepatocellular carcinoma cell line Hepa 1-6 was used as a model in this study .
	manualset3
216430	1	419977	7	NULL	NULL	0	NULL	 method 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The method involves the combined use of stable isotopically labeled internal standards ( DDVP-d ( 6 ) , malathion-d ( 10 ) , carbaryl-d ( 7 ) , and 2 , 4-D-d ( 5 ) ) and a multiple reaction monitoring technique .
	manualset3
216431	2	419977	7	NULL	NULL	0	NULL	combined use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method involves the combined use of stable isotopically labeled internal standards ( DDVP-d ( 6 ) , malathion-d ( 10 ) , carbaryl-d ( 7 ) , and 2 , 4-D-d ( 5 ) ) and a multiple reaction monitoring technique .
	manualset3
216432	3	419977	7	NULL	NULL	0	NULL	stable isotopically labeled internal standards	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method involves the combined use of stable isotopically labeled internal standards ( DDVP-d ( 6 ) , malathion-d ( 10 ) , carbaryl-d ( 7 ) , and 2 , 4-D-d ( 5 ) ) and a multiple reaction monitoring technique .
	manualset3
216433	4	419977	7	NULL	NULL	0	NULL	DDVP-d ( 6 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The method involves the combined use of stable isotopically labeled internal standards ( DDVP-d ( 6 ) , malathion-d ( 10 ) , carbaryl-d ( 7 ) , and 2 , 4-D-d ( 5 ) ) and a multiple reaction monitoring technique .
	manualset3
216434	5	419977	7	NULL	NULL	0	NULL	malathion-d ( 10 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The method involves the combined use of stable isotopically labeled internal standards ( DDVP-d ( 6 ) , malathion-d ( 10 ) , carbaryl-d ( 7 ) , and 2 , 4-D-d ( 5 ) ) and a multiple reaction monitoring technique .
	manualset3
216435	6	419977	7	NULL	NULL	0	NULL	carbaryl-d ( 7 ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The method involves the combined use of stable isotopically labeled internal standards ( DDVP-d ( 6 ) , malathion-d ( 10 ) , carbaryl-d ( 7 ) , and 2 , 4-D-d ( 5 ) ) and a multiple reaction monitoring technique .
	manualset3
216436	7	419977	7	NULL	NULL	0	NULL	 2 , 4-D-d ( 5 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The method involves the combined use of stable isotopically labeled internal standards ( DDVP-d ( 6 ) , malathion-d ( 10 ) , carbaryl-d ( 7 ) , and 2 , 4-D-d ( 5 ) ) and a multiple reaction monitoring technique .
	manualset3
216437	8	419977	7	NULL	NULL	0	NULL	multiple reaction monitoring technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method involves the combined use of stable isotopically labeled internal standards ( DDVP-d ( 6 ) , malathion-d ( 10 ) , carbaryl-d ( 7 ) , and 2 , 4-D-d ( 5 ) ) and a multiple reaction monitoring technique .
	manualset3
216438	1	419978	7	NULL	NULL	NULL	NULL	P-A-I-N MMPI classification system	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The P-A-I-N MMPI classification system : a critical review .
	manualset3
216439	2	419978	7	NULL	NULL	0	NULL	critical review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The P-A-I-N MMPI classification system : a critical review .
	manualset3
216440	1	419979	7	NULL	NULL	0	NULL	Acquired resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acquired resistance to fatty acids and sulfanilamide of certain trichophyton-strains .
	manualset3
216441	2	419979	7	NULL	NULL	0	NULL	 fatty acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Acquired resistance to fatty acids and sulfanilamide of certain trichophyton-strains .
	manualset3
216442	3	419979	7	NULL	NULL	0	NULL	sulfanilamide 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Acquired resistance to fatty acids and sulfanilamide of certain trichophyton-strains .
	manualset3
216443	4	419979	7	NULL	NULL	0	NULL	trichophyton-strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Acquired resistance to fatty acids and sulfanilamide of certain trichophyton-strains .
	manualset3
216444	1	419980	7	NULL	NULL	0	NULL	 majority	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the majority of stored glucocerebroside in GC is of erythrocyte origin , apparent erythrophagocytosis by GC in bone marrow is an unusual finding .
	manualset3
216445	2	419980	7	NULL	NULL	0	NULL	stored glucocerebroside	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the majority of stored glucocerebroside in GC is of erythrocyte origin , apparent erythrophagocytosis by GC in bone marrow is an unusual finding .
	manualset3
216446	3	419980	7	NULL	NULL	0	NULL	GC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the majority of stored glucocerebroside in GC is of erythrocyte origin , apparent erythrophagocytosis by GC in bone marrow is an unusual finding .
	manualset3
216447	4	419980	7	NULL	NULL	0	NULL	erythrocyte origin	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the majority of stored glucocerebroside in GC is of erythrocyte origin , apparent erythrophagocytosis by GC in bone marrow is an unusual finding .
	manualset3
216448	5	419980	7	NULL	NULL	0	NULL	erythrophagocytosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the majority of stored glucocerebroside in GC is of erythrocyte origin , apparent erythrophagocytosis by GC in bone marrow is an unusual finding .
	manualset3
216449	6	419980	7	NULL	NULL	0	NULL	GC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the majority of stored glucocerebroside in GC is of erythrocyte origin , apparent erythrophagocytosis by GC in bone marrow is an unusual finding .
	manualset3
216450	7	419980	7	NULL	NULL	0	NULL	bone marrow	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the majority of stored glucocerebroside in GC is of erythrocyte origin , apparent erythrophagocytosis by GC in bone marrow is an unusual finding .
	manualset3
216451	8	419980	7	NULL	NULL	0	NULL	 unusual finding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the majority of stored glucocerebroside in GC is of erythrocyte origin , apparent erythrophagocytosis by GC in bone marrow is an unusual finding .
	manualset3
216452	1	419981	7	NULL	NULL	0	NULL	phagocytic neutrophils	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Clearing phagocytic neutrophils by triggering apoptosis is an essential process for controlling inflammation .
	manualset3
216453	2	419981	7	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Clearing phagocytic neutrophils by triggering apoptosis is an essential process for controlling inflammation .
	manualset3
216454	3	419981	7	NULL	NULL	0	NULL	essential process	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Clearing phagocytic neutrophils by triggering apoptosis is an essential process for controlling inflammation .
	manualset3
216455	4	419981	7	NULL	NULL	0	NULL	 inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Clearing phagocytic neutrophils by triggering apoptosis is an essential process for controlling inflammation .
	manualset3
216456	1	419982	7	NULL	NULL	0	NULL	Results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of 104 arthrotomography scans with contrast of temporomandibular joints of 71 patients are used to define normal arthrography criteria ( 15.4 % of cases ) .
	manualset3
216457	2	419982	7	NULL	NULL	0	NULL	104 arthrotomography scans	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of 104 arthrotomography scans with contrast of temporomandibular joints of 71 patients are used to define normal arthrography criteria ( 15.4 % of cases ) .
	manualset3
216458	3	419982	7	NULL	NULL	0	NULL	temporomandibular joints	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of 104 arthrotomography scans with contrast of temporomandibular joints of 71 patients are used to define normal arthrography criteria ( 15.4 % of cases ) .
	manualset3
216459	4	419982	7	NULL	NULL	0	NULL	71 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of 104 arthrotomography scans with contrast of temporomandibular joints of 71 patients are used to define normal arthrography criteria ( 15.4 % of cases ) .
	manualset3
216460	5	419982	7	NULL	NULL	0	NULL	normal arthrography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of 104 arthrotomography scans with contrast of temporomandibular joints of 71 patients are used to define normal arthrography criteria ( 15.4 % of cases ) .
	manualset3
216461	6	419982	7	NULL	NULL	0	NULL	15.4 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of 104 arthrotomography scans with contrast of temporomandibular joints of 71 patients are used to define normal arthrography criteria ( 15.4 % of cases ) .
	manualset3
216462	7	419982	7	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results of 104 arthrotomography scans with contrast of temporomandibular joints of 71 patients are used to define normal arthrography criteria ( 15.4 % of cases ) .
	manualset3
216463	1	419983	7	NULL	NULL	0	NULL	Prognostic value	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic value of a bone resorption marker , tartrate-resistant acid phosphatase isoform 5b ( TRACP 5b ) , and two matrix metalloproteinases ( MMP-2 and MMP-9 ) was compared with the standard clinical analyses of total alkaline phosphatase ( tALP ) and prostate-specific antigen ( PSA ) , in prostate cancer ( PC ) patients with ( BM + ) or without ( BM - ) bone metastases .
	manualset3
216464	2	419983	7	NULL	NULL	0	NULL	bone resorption marker	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic value of a bone resorption marker , tartrate-resistant acid phosphatase isoform 5b ( TRACP 5b ) , and two matrix metalloproteinases ( MMP-2 and MMP-9 ) was compared with the standard clinical analyses of total alkaline phosphatase ( tALP ) and prostate-specific antigen ( PSA ) , in prostate cancer ( PC ) patients with ( BM + ) or without ( BM - ) bone metastases .
	manualset3
216465	3	419983	7	NULL	NULL	0	NULL	 tartrate-resistant acid phosphatase isoform 5b ( TRACP 5b )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic value of a bone resorption marker , tartrate-resistant acid phosphatase isoform 5b ( TRACP 5b ) , and two matrix metalloproteinases ( MMP-2 and MMP-9 ) was compared with the standard clinical analyses of total alkaline phosphatase ( tALP ) and prostate-specific antigen ( PSA ) , in prostate cancer ( PC ) patients with ( BM + ) or without ( BM - ) bone metastases .
	manualset3
216466	4	419983	7	NULL	NULL	0	NULL	two matrix metalloproteinases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic value of a bone resorption marker , tartrate-resistant acid phosphatase isoform 5b ( TRACP 5b ) , and two matrix metalloproteinases ( MMP-2 and MMP-9 ) was compared with the standard clinical analyses of total alkaline phosphatase ( tALP ) and prostate-specific antigen ( PSA ) , in prostate cancer ( PC ) patients with ( BM + ) or without ( BM - ) bone metastases .
	manualset3
216467	5	419983	7	NULL	NULL	0	NULL	MMP-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic value of a bone resorption marker , tartrate-resistant acid phosphatase isoform 5b ( TRACP 5b ) , and two matrix metalloproteinases ( MMP-2 and MMP-9 ) was compared with the standard clinical analyses of total alkaline phosphatase ( tALP ) and prostate-specific antigen ( PSA ) , in prostate cancer ( PC ) patients with ( BM + ) or without ( BM - ) bone metastases .
	manualset3
216468	6	419983	7	NULL	NULL	0	NULL	MMP-9	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic value of a bone resorption marker , tartrate-resistant acid phosphatase isoform 5b ( TRACP 5b ) , and two matrix metalloproteinases ( MMP-2 and MMP-9 ) was compared with the standard clinical analyses of total alkaline phosphatase ( tALP ) and prostate-specific antigen ( PSA ) , in prostate cancer ( PC ) patients with ( BM + ) or without ( BM - ) bone metastases .
	manualset3
216469	7	419983	7	NULL	NULL	0	NULL	standard clinical analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic value of a bone resorption marker , tartrate-resistant acid phosphatase isoform 5b ( TRACP 5b ) , and two matrix metalloproteinases ( MMP-2 and MMP-9 ) was compared with the standard clinical analyses of total alkaline phosphatase ( tALP ) and prostate-specific antigen ( PSA ) , in prostate cancer ( PC ) patients with ( BM + ) or without ( BM - ) bone metastases .
	manualset3
216470	8	419983	7	NULL	NULL	0	NULL	total alkaline phosphatase ( tALP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic value of a bone resorption marker , tartrate-resistant acid phosphatase isoform 5b ( TRACP 5b ) , and two matrix metalloproteinases ( MMP-2 and MMP-9 ) was compared with the standard clinical analyses of total alkaline phosphatase ( tALP ) and prostate-specific antigen ( PSA ) , in prostate cancer ( PC ) patients with ( BM + ) or without ( BM - ) bone metastases .
	manualset3
216471	9	419983	7	NULL	NULL	0	NULL	 prostate-specific antigen ( PSA )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic value of a bone resorption marker , tartrate-resistant acid phosphatase isoform 5b ( TRACP 5b ) , and two matrix metalloproteinases ( MMP-2 and MMP-9 ) was compared with the standard clinical analyses of total alkaline phosphatase ( tALP ) and prostate-specific antigen ( PSA ) , in prostate cancer ( PC ) patients with ( BM + ) or without ( BM - ) bone metastases .
	manualset3
216472	10	419983	7	NULL	NULL	0	NULL	prostate cancer ( PC )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic value of a bone resorption marker , tartrate-resistant acid phosphatase isoform 5b ( TRACP 5b ) , and two matrix metalloproteinases ( MMP-2 and MMP-9 ) was compared with the standard clinical analyses of total alkaline phosphatase ( tALP ) and prostate-specific antigen ( PSA ) , in prostate cancer ( PC ) patients with ( BM + ) or without ( BM - ) bone metastases .
	manualset3
216473	11	419983	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic value of a bone resorption marker , tartrate-resistant acid phosphatase isoform 5b ( TRACP 5b ) , and two matrix metalloproteinases ( MMP-2 and MMP-9 ) was compared with the standard clinical analyses of total alkaline phosphatase ( tALP ) and prostate-specific antigen ( PSA ) , in prostate cancer ( PC ) patients with ( BM + ) or without ( BM - ) bone metastases .
	manualset3
216474	12	419983	7	NULL	NULL	0	NULL	( BM + ) bone metastases	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic value of a bone resorption marker , tartrate-resistant acid phosphatase isoform 5b ( TRACP 5b ) , and two matrix metalloproteinases ( MMP-2 and MMP-9 ) was compared with the standard clinical analyses of total alkaline phosphatase ( tALP ) and prostate-specific antigen ( PSA ) , in prostate cancer ( PC ) patients with ( BM + ) or without ( BM - ) bone metastases .
	manualset3
216475	13	419983	7	NULL	NULL	0	NULL	( BM - ) bone metastases .	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Prognostic value of a bone resorption marker , tartrate-resistant acid phosphatase isoform 5b ( TRACP 5b ) , and two matrix metalloproteinases ( MMP-2 and MMP-9 ) was compared with the standard clinical analyses of total alkaline phosphatase ( tALP ) and prostate-specific antigen ( PSA ) , in prostate cancer ( PC ) patients with ( BM + ) or without ( BM - ) bone metastases .
	manualset3
216476	1	419984	7	NULL	NULL	0	NULL	mol-ecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In each mol-ecule , four penta-fluoro-benzoate anions bridge the quadruply bonded Mo ( 2 ) ( 4 + ) unit that is , in addition , axially coordinated by two O atoms of tetra-hydro-furan ( THF ) mol-ecules .
	manualset3
216477	2	419984	7	NULL	NULL	0	NULL	four penta-fluoro-benzoate anions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In each mol-ecule , four penta-fluoro-benzoate anions bridge the quadruply bonded Mo ( 2 ) ( 4 + ) unit that is , in addition , axially coordinated by two O atoms of tetra-hydro-furan ( THF ) mol-ecules .
	manualset3
216478	3	419984	7	NULL	NULL	0	NULL	Mo ( 2 ) ( 4 + ) unit	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In each mol-ecule , four penta-fluoro-benzoate anions bridge the quadruply bonded Mo ( 2 ) ( 4 + ) unit that is , in addition , axially coordinated by two O atoms of tetra-hydro-furan ( THF ) mol-ecules .
	manualset3
216479	4	419984	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In each mol-ecule , four penta-fluoro-benzoate anions bridge the quadruply bonded Mo ( 2 ) ( 4 + ) unit that is , in addition , axially coordinated by two O atoms of tetra-hydro-furan ( THF ) mol-ecules .
	manualset3
216480	5	419984	7	NULL	NULL	0	NULL	two O atoms 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	In each mol-ecule , four penta-fluoro-benzoate anions bridge the quadruply bonded Mo ( 2 ) ( 4 + ) unit that is , in addition , axially coordinated by two O atoms of tetra-hydro-furan ( THF ) mol-ecules .
	manualset3
216481	6	419984	7	NULL	NULL	0	NULL	tetra-hydro-furan ( THF ) mol-ecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In each mol-ecule , four penta-fluoro-benzoate anions bridge the quadruply bonded Mo ( 2 ) ( 4 + ) unit that is , in addition , axially coordinated by two O atoms of tetra-hydro-furan ( THF ) mol-ecules .
	manualset3
216482	1	419985	7	NULL	NULL	0	NULL	PDT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	However , during PDT , there are many difficulties , so it is not possible to excite the photosensitizer using a laser , a source of light at the wavelengths specific to the photosensitizer ( in visible region of the spectrum ) .
	manualset3
216483	2	419985	7	NULL	NULL	0	NULL	photosensitizer	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	However , during PDT , there are many difficulties , so it is not possible to excite the photosensitizer using a laser , a source of light at the wavelengths specific to the photosensitizer ( in visible region of the spectrum ) .
	manualset3
216484	3	419985	7	NULL	NULL	0	NULL	 laser	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , during PDT , there are many difficulties , so it is not possible to excite the photosensitizer using a laser , a source of light at the wavelengths specific to the photosensitizer ( in visible region of the spectrum ) .
	manualset3
216485	4	419985	7	NULL	NULL	0	NULL	source of light 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , during PDT , there are many difficulties , so it is not possible to excite the photosensitizer using a laser , a source of light at the wavelengths specific to the photosensitizer ( in visible region of the spectrum ) .
	manualset3
216486	5	419985	7	NULL	NULL	0	NULL	wavelengths	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , during PDT , there are many difficulties , so it is not possible to excite the photosensitizer using a laser , a source of light at the wavelengths specific to the photosensitizer ( in visible region of the spectrum ) .
	manualset3
216487	6	419985	7	NULL	NULL	0	NULL	photosensitizer	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	However , during PDT , there are many difficulties , so it is not possible to excite the photosensitizer using a laser , a source of light at the wavelengths specific to the photosensitizer ( in visible region of the spectrum ) .
	manualset3
216488	7	419985	7	NULL	NULL	0	NULL	visible region	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , during PDT , there are many difficulties , so it is not possible to excite the photosensitizer using a laser , a source of light at the wavelengths specific to the photosensitizer ( in visible region of the spectrum ) .
	manualset3
216489	8	419985	7	NULL	NULL	0	NULL	spectrum 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	However , during PDT , there are many difficulties , so it is not possible to excite the photosensitizer using a laser , a source of light at the wavelengths specific to the photosensitizer ( in visible region of the spectrum ) .
	manualset3
216490	1	419986	7	NULL	NULL	0	NULL	survey data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These survey data suggest that the prevalence of CKD has increased between 1988-1994 and 1999-2004 .
	manualset3
216491	2	419986	7	NULL	NULL	0	NULL	prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These survey data suggest that the prevalence of CKD has increased between 1988-1994 and 1999-2004 .
	manualset3
216492	3	419986	7	NULL	NULL	0	NULL	CKD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These survey data suggest that the prevalence of CKD has increased between 1988-1994 and 1999-2004 .
	manualset3
216493	4	419986	7	NULL	NULL	0	NULL	1988-1994	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	These survey data suggest that the prevalence of CKD has increased between 1988-1994 and 1999-2004 .
	manualset3
216494	5	419986	7	NULL	NULL	0	NULL	1999-2004	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	These survey data suggest that the prevalence of CKD has increased between 1988-1994 and 1999-2004 .
	manualset3
216495	1	419987	7	NULL	NULL	0	NULL	arterial stiffness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the marked increase of arterial and cardiac stiffness with aging can maintain ventricular-vascular coupling within a normal range , it does have detrimental effects on hemodynamic stability and cardiac reserve .
	manualset3
216496	2	419987	7	NULL	NULL	0	NULL	cardiac stiffness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the marked increase of arterial and cardiac stiffness with aging can maintain ventricular-vascular coupling within a normal range , it does have detrimental effects on hemodynamic stability and cardiac reserve .
	manualset3
216497	3	419987	7	NULL	NULL	0	NULL	aging	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the marked increase of arterial and cardiac stiffness with aging can maintain ventricular-vascular coupling within a normal range , it does have detrimental effects on hemodynamic stability and cardiac reserve .
	manualset3
216498	4	419987	7	NULL	NULL	0	NULL	ventricular-vascular coupling	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the marked increase of arterial and cardiac stiffness with aging can maintain ventricular-vascular coupling within a normal range , it does have detrimental effects on hemodynamic stability and cardiac reserve .
	manualset3
216499	5	419987	7	NULL	NULL	0	NULL	 normal range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the marked increase of arterial and cardiac stiffness with aging can maintain ventricular-vascular coupling within a normal range , it does have detrimental effects on hemodynamic stability and cardiac reserve .
	manualset3
216500	6	419987	7	NULL	NULL	0	NULL	detrimental effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the marked increase of arterial and cardiac stiffness with aging can maintain ventricular-vascular coupling within a normal range , it does have detrimental effects on hemodynamic stability and cardiac reserve .
	manualset3
216501	7	419987	7	NULL	NULL	0	NULL	 hemodynamic stability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the marked increase of arterial and cardiac stiffness with aging can maintain ventricular-vascular coupling within a normal range , it does have detrimental effects on hemodynamic stability and cardiac reserve .
	manualset3
216502	8	419987	7	NULL	NULL	0	NULL	cardiac reserve 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the marked increase of arterial and cardiac stiffness with aging can maintain ventricular-vascular coupling within a normal range , it does have detrimental effects on hemodynamic stability and cardiac reserve .
	manualset3
217440	9	419987	7	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the marked increase of arterial and cardiac stiffness with aging can maintain ventricular-vascular coupling within a normal range , it does have detrimental effects on hemodynamic stability and cardiac reserve .
	manualset3
216503	1	419988	7	NULL	NULL	0	NULL	 inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	During inflammation polymorphonuclear cells ( PMNs ) are exposed to agonistic stimuli including activated complement , kallikrein , arachidonic acid metabolites , monokines , and platelet-activating factor ( PAF ) .
	manualset3
216504	2	419988	7	NULL	NULL	0	NULL	polymorphonuclear cells ( PMNs ) 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	During inflammation polymorphonuclear cells ( PMNs ) are exposed to agonistic stimuli including activated complement , kallikrein , arachidonic acid metabolites , monokines , and platelet-activating factor ( PAF ) .
	manualset3
216505	3	419988	7	NULL	NULL	0	NULL	agonistic stimuli	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	During inflammation polymorphonuclear cells ( PMNs ) are exposed to agonistic stimuli including activated complement , kallikrein , arachidonic acid metabolites , monokines , and platelet-activating factor ( PAF ) .
	manualset3
216506	4	419988	7	NULL	NULL	0	NULL	activated complement	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	During inflammation polymorphonuclear cells ( PMNs ) are exposed to agonistic stimuli including activated complement , kallikrein , arachidonic acid metabolites , monokines , and platelet-activating factor ( PAF ) .
	manualset3
216507	5	419988	7	NULL	NULL	0	NULL	kallikrein	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	During inflammation polymorphonuclear cells ( PMNs ) are exposed to agonistic stimuli including activated complement , kallikrein , arachidonic acid metabolites , monokines , and platelet-activating factor ( PAF ) .
	manualset3
216508	6	419988	7	NULL	NULL	0	NULL	arachidonic acid metabolites	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	During inflammation polymorphonuclear cells ( PMNs ) are exposed to agonistic stimuli including activated complement , kallikrein , arachidonic acid metabolites , monokines , and platelet-activating factor ( PAF ) .
	manualset3
216509	7	419988	7	NULL	NULL	0	NULL	monokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	During inflammation polymorphonuclear cells ( PMNs ) are exposed to agonistic stimuli including activated complement , kallikrein , arachidonic acid metabolites , monokines , and platelet-activating factor ( PAF ) .
	manualset3
216510	8	419988	7	NULL	NULL	0	NULL	platelet-activating factor ( PAF )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	During inflammation polymorphonuclear cells ( PMNs ) are exposed to agonistic stimuli including activated complement , kallikrein , arachidonic acid metabolites , monokines , and platelet-activating factor ( PAF ) .
	manualset3
216511	1	419989	7	NULL	NULL	0	NULL	Effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of combined chloramphenicol and neomycin therapy on the clinical and bacteriological therapy of infantile shigelloses ) .
	manualset3
216512	2	419989	7	NULL	NULL	0	NULL	chloramphenicol therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of combined chloramphenicol and neomycin therapy on the clinical and bacteriological therapy of infantile shigelloses ) .
	manualset3
216513	3	419989	7	NULL	NULL	0	NULL	neomycin therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of combined chloramphenicol and neomycin therapy on the clinical and bacteriological therapy of infantile shigelloses ) .
	manualset3
216514	4	419989	7	NULL	NULL	0	NULL	clinical therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of combined chloramphenicol and neomycin therapy on the clinical and bacteriological therapy of infantile shigelloses ) .
	manualset3
216515	5	419989	7	NULL	NULL	0	NULL	bacteriological therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of combined chloramphenicol and neomycin therapy on the clinical and bacteriological therapy of infantile shigelloses ) .
	manualset3
216516	6	419989	7	NULL	NULL	0	NULL	infantile shigelloses	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of combined chloramphenicol and neomycin therapy on the clinical and bacteriological therapy of infantile shigelloses ) .
	manualset3
216517	1	419990	7	NULL	NULL	0	NULL	X-ray diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( X-ray diagnosis of organic stenosis of the outlet of the stomach ) .
	manualset3
216518	2	419990	7	NULL	NULL	0	NULL	organic stenosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( X-ray diagnosis of organic stenosis of the outlet of the stomach ) .
	manualset3
216519	3	419990	7	NULL	NULL	0	NULL	outlet	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( X-ray diagnosis of organic stenosis of the outlet of the stomach ) .
	manualset3
216520	4	419990	7	NULL	NULL	0	NULL	 stomach 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( X-ray diagnosis of organic stenosis of the outlet of the stomach ) .
	manualset3
216521	1	419991	7	NULL	NULL	0	NULL	new medical management information system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	And it 's putting the finishing touches on a sophisticated new medical management information system to track cost , quality and patient satisfaction .
	manualset3
216522	2	419991	7	NULL	NULL	0	NULL	 cost	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	And it 's putting the finishing touches on a sophisticated new medical management information system to track cost , quality and patient satisfaction .
	manualset3
216523	3	419991	7	NULL	NULL	0	NULL	quality	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	And it 's putting the finishing touches on a sophisticated new medical management information system to track cost , quality and patient satisfaction .
	manualset3
216524	4	419991	7	NULL	NULL	0	NULL	patient satisfaction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	And it 's putting the finishing touches on a sophisticated new medical management information system to track cost , quality and patient satisfaction .
	manualset3
216525	1	419992	7	NULL	NULL	0	NULL	Renal excretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal excretion of oxalate in patients with chronic renal failure or nephrolithiasis .
	manualset3
216526	2	419992	7	NULL	NULL	0	NULL	oxalate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal excretion of oxalate in patients with chronic renal failure or nephrolithiasis .
	manualset3
216527	3	419992	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal excretion of oxalate in patients with chronic renal failure or nephrolithiasis .
	manualset3
216528	4	419992	7	NULL	NULL	0	NULL	chronic renal failure 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal excretion of oxalate in patients with chronic renal failure or nephrolithiasis .
	manualset3
216529	5	419992	7	NULL	NULL	0	NULL	nephrolithiasis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Renal excretion of oxalate in patients with chronic renal failure or nephrolithiasis .
	manualset3
216530	1	419993	7	NULL	NULL	0	NULL	PACAP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PACAP increased ( P & lt ; 0.001 ) both the number of follistatin-expressing cells as well as the number of grains per cell in both gonadotrophs and folliculostellate cells , while GnRH only affected ( P = 0.01 ) gonadotrophs .
	manualset3
216531	2	419993	7	NULL	NULL	0	NULL	P & lt ; 0.001	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PACAP increased ( P & lt ; 0.001 ) both the number of follistatin-expressing cells as well as the number of grains per cell in both gonadotrophs and folliculostellate cells , while GnRH only affected ( P = 0.01 ) gonadotrophs .
	manualset3
216532	3	419993	7	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PACAP increased ( P & lt ; 0.001 ) both the number of follistatin-expressing cells as well as the number of grains per cell in both gonadotrophs and folliculostellate cells , while GnRH only affected ( P = 0.01 ) gonadotrophs .
	manualset3
216533	4	419993	7	NULL	NULL	0	NULL	 follistatin-expressing cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	PACAP increased ( P & lt ; 0.001 ) both the number of follistatin-expressing cells as well as the number of grains per cell in both gonadotrophs and folliculostellate cells , while GnRH only affected ( P = 0.01 ) gonadotrophs .
	manualset3
216534	5	419993	7	NULL	NULL	NULL	NULL	number 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	PACAP increased ( P & lt ; 0.001 ) both the number of follistatin-expressing cells as well as the number of grains per cell in both gonadotrophs and folliculostellate cells , while GnRH only affected ( P = 0.01 ) gonadotrophs .
	manualset3
216535	6	419993	7	NULL	NULL	0	NULL	grains per cell 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PACAP increased ( P & lt ; 0.001 ) both the number of follistatin-expressing cells as well as the number of grains per cell in both gonadotrophs and folliculostellate cells , while GnRH only affected ( P = 0.01 ) gonadotrophs .
	manualset3
216536	7	419993	7	NULL	NULL	0	NULL	gonadotrophs cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	PACAP increased ( P & lt ; 0.001 ) both the number of follistatin-expressing cells as well as the number of grains per cell in both gonadotrophs and folliculostellate cells , while GnRH only affected ( P = 0.01 ) gonadotrophs .
	manualset3
216537	8	419993	7	NULL	NULL	0	NULL	folliculostellate cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	PACAP increased ( P & lt ; 0.001 ) both the number of follistatin-expressing cells as well as the number of grains per cell in both gonadotrophs and folliculostellate cells , while GnRH only affected ( P = 0.01 ) gonadotrophs .
	manualset3
216538	9	419993	7	NULL	NULL	NULL	NULL	GnRH	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	PACAP increased ( P & lt ; 0.001 ) both the number of follistatin-expressing cells as well as the number of grains per cell in both gonadotrophs and folliculostellate cells , while GnRH only affected ( P = 0.01 ) gonadotrophs .
	manualset3
216539	10	419993	7	NULL	NULL	NULL	NULL	gonadotrophs	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	PACAP increased ( P & lt ; 0.001 ) both the number of follistatin-expressing cells as well as the number of grains per cell in both gonadotrophs and folliculostellate cells , while GnRH only affected ( P = 0.01 ) gonadotrophs .
	manualset3
217441	11	419993	7	NULL	NULL	0	NULL	 P = 0.01	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PACAP increased ( P & lt ; 0.001 ) both the number of follistatin-expressing cells as well as the number of grains per cell in both gonadotrophs and folliculostellate cells , while GnRH only affected ( P = 0.01 ) gonadotrophs .
	manualset3
216540	1	419994	7	NULL	NULL	0	NULL	Social gradients	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Social gradients in binge drinking and abstaining : trends in a cohort of British adults .
	manualset3
216541	2	419994	7	NULL	NULL	0	NULL	binge drinking	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Social gradients in binge drinking and abstaining : trends in a cohort of British adults .
	manualset3
216542	3	419994	7	NULL	NULL	0	NULL	abstaining	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Social gradients in binge drinking and abstaining : trends in a cohort of British adults .
	manualset3
216543	4	419994	7	NULL	NULL	0	NULL	trends	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Social gradients in binge drinking and abstaining : trends in a cohort of British adults .
	manualset3
216544	5	419994	7	NULL	NULL	0	NULL	cohort	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Social gradients in binge drinking and abstaining : trends in a cohort of British adults .
	manualset3
216545	6	419994	7	NULL	NULL	0	NULL	British adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Social gradients in binge drinking and abstaining : trends in a cohort of British adults .
	manualset3
216546	1	419995	7	NULL	NULL	0	NULL	Safety	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety of 5-HT reuptake inhibitors .
	manualset3
216547	2	419995	7	NULL	NULL	NULL	NULL	5-HT reuptake	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Safety of 5-HT reuptake inhibitors .
	manualset3
216548	3	419995	7	NULL	NULL	0	NULL	inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Safety of 5-HT reuptake inhibitors .
	manualset3
216549	1	419996	7	NULL	NULL	0	NULL	mechanism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the mechanism of choroidal expansion is unknown , it might involve either a increased routing of aqueous humor into the uveoscleral outflow or osmotically generated water movement into the choroid .
	manualset3
216550	2	419996	7	NULL	NULL	0	NULL	choroidal expansion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the mechanism of choroidal expansion is unknown , it might involve either a increased routing of aqueous humor into the uveoscleral outflow or osmotically generated water movement into the choroid .
	manualset3
216551	3	419996	7	NULL	NULL	0	NULL	increased routing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the mechanism of choroidal expansion is unknown , it might involve either a increased routing of aqueous humor into the uveoscleral outflow or osmotically generated water movement into the choroid .
	manualset3
216552	4	419996	7	NULL	NULL	0	NULL	aqueous humor	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the mechanism of choroidal expansion is unknown , it might involve either a increased routing of aqueous humor into the uveoscleral outflow or osmotically generated water movement into the choroid .
	manualset3
216553	5	419996	7	NULL	NULL	0	NULL	uveoscleral outflow	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the mechanism of choroidal expansion is unknown , it might involve either a increased routing of aqueous humor into the uveoscleral outflow or osmotically generated water movement into the choroid .
	manualset3
216554	6	419996	7	NULL	NULL	0	NULL	osmotically generated water movement	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the mechanism of choroidal expansion is unknown , it might involve either a increased routing of aqueous humor into the uveoscleral outflow or osmotically generated water movement into the choroid .
	manualset3
216555	7	419996	7	NULL	NULL	0	NULL	choroid	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the mechanism of choroidal expansion is unknown , it might involve either a increased routing of aqueous humor into the uveoscleral outflow or osmotically generated water movement into the choroid .
	manualset3
216556	1	419997	7	NULL	NULL	0	NULL	TRPV1 cation channel	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The TRPV1 cation channel is a member of the thermo-TRP family of ionic channels activated by noxious heat and various endogenous mediators .
	manualset3
216557	2	419997	7	NULL	NULL	0	NULL	member	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The TRPV1 cation channel is a member of the thermo-TRP family of ionic channels activated by noxious heat and various endogenous mediators .
	manualset3
216558	3	419997	7	NULL	NULL	0	NULL	thermo-TRP family	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The TRPV1 cation channel is a member of the thermo-TRP family of ionic channels activated by noxious heat and various endogenous mediators .
	manualset3
216559	4	419997	7	NULL	NULL	0	NULL	ionic channels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The TRPV1 cation channel is a member of the thermo-TRP family of ionic channels activated by noxious heat and various endogenous mediators .
	manualset3
216560	5	419997	7	NULL	NULL	0	NULL	noxious heat mediators	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The TRPV1 cation channel is a member of the thermo-TRP family of ionic channels activated by noxious heat and various endogenous mediators .
	manualset3
216561	6	419997	7	NULL	NULL	0	NULL	endogenous mediators	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The TRPV1 cation channel is a member of the thermo-TRP family of ionic channels activated by noxious heat and various endogenous mediators .
	manualset3
216562	1	419998	7	NULL	NULL	0	NULL	 prostate cancers ( PCa 's )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Because prostate cancers ( PCa 's ) rarely grow as xenografts , indentifying PCa repopulating cells has not been possible .
	manualset3
216563	2	419998	7	NULL	NULL	0	NULL	xenografts 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Because prostate cancers ( PCa 's ) rarely grow as xenografts , indentifying PCa repopulating cells has not been possible .
	manualset3
216564	3	419998	7	NULL	NULL	0	NULL	PCa repopulating cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Because prostate cancers ( PCa 's ) rarely grow as xenografts , indentifying PCa repopulating cells has not been possible .
	manualset3
216565	1	419999	7	NULL	NULL	0	NULL	Co-administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-administration of BSO and DEM ( 1000 mg/kg , 0.6 mL/kg , respectively ) substantially depleted gill GSH and eliminated detectable liver GSH .
	manualset3
216566	2	419999	7	NULL	NULL	0	NULL	BSO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-administration of BSO and DEM ( 1000 mg/kg , 0.6 mL/kg , respectively ) substantially depleted gill GSH and eliminated detectable liver GSH .
	manualset3
216567	3	419999	7	NULL	NULL	0	NULL	DEM	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-administration of BSO and DEM ( 1000 mg/kg , 0.6 mL/kg , respectively ) substantially depleted gill GSH and eliminated detectable liver GSH .
	manualset3
216568	4	419999	7	NULL	NULL	0	NULL	1000 mg/kg	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-administration of BSO and DEM ( 1000 mg/kg , 0.6 mL/kg , respectively ) substantially depleted gill GSH and eliminated detectable liver GSH .
	manualset3
216569	5	419999	7	NULL	NULL	0	NULL	 0.6 mL/kg	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-administration of BSO and DEM ( 1000 mg/kg , 0.6 mL/kg , respectively ) substantially depleted gill GSH and eliminated detectable liver GSH .
	manualset3
216570	6	419999	7	NULL	NULL	0	NULL	gill GSH	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-administration of BSO and DEM ( 1000 mg/kg , 0.6 mL/kg , respectively ) substantially depleted gill GSH and eliminated detectable liver GSH .
	manualset3
216571	7	419999	7	NULL	NULL	0	NULL	liver GSH	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-administration of BSO and DEM ( 1000 mg/kg , 0.6 mL/kg , respectively ) substantially depleted gill GSH and eliminated detectable liver GSH .
	manualset3
216572	1	420000	7	NULL	NULL	0	NULL	Economic adjustment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Economic adjustment of migrants in the city : the Jakarta experience .
	manualset3
216573	2	420000	7	NULL	NULL	0	NULL	 migrants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Economic adjustment of migrants in the city : the Jakarta experience .
	manualset3
216574	3	420000	7	NULL	NULL	0	NULL	city	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Economic adjustment of migrants in the city : the Jakarta experience .
	manualset3
216575	4	420000	7	NULL	NULL	0	NULL	Jakarta experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Economic adjustment of migrants in the city : the Jakarta experience .
	manualset3
216576	1	420001	7	NULL	NULL	0	NULL	Endocrine disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Endocrine disorders render rats hyporeactive to non-steroidal but not to steroidal anti-inflammatory drugs .
	manualset3
216577	2	420001	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Endocrine disorders render rats hyporeactive to non-steroidal but not to steroidal anti-inflammatory drugs .
	manualset3
216578	3	420001	7	NULL	NULL	NULL	NULL	non-steroidal anti-inflammatory drugs	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Endocrine disorders render rats hyporeactive to non-steroidal but not to steroidal anti-inflammatory drugs .
	manualset3
216579	4	420001	7	NULL	NULL	0	NULL	steroidal anti-inflammatory drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Endocrine disorders render rats hyporeactive to non-steroidal but not to steroidal anti-inflammatory drugs .
	manualset3
216580	1	420002	7	NULL	NULL	0	NULL	fibroblast growth factor receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Importance of fibroblast growth factor receptor in neovascularization and tumor escape from antiangiogenic therapy .
	manualset3
216581	2	420002	7	NULL	NULL	0	NULL	neovascularization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Importance of fibroblast growth factor receptor in neovascularization and tumor escape from antiangiogenic therapy .
	manualset3
216582	3	420002	7	NULL	NULL	0	NULL	tumor escape	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Importance of fibroblast growth factor receptor in neovascularization and tumor escape from antiangiogenic therapy .
	manualset3
216583	4	420002	7	NULL	NULL	0	NULL	antiangiogenic therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Importance of fibroblast growth factor receptor in neovascularization and tumor escape from antiangiogenic therapy .
	manualset3
216584	1	420003	7	NULL	NULL	0	NULL	SCP1 overexpression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SCP1 overexpression also counteracts the inhibitory effect of epidermal growth factor on TGF-beta-induced p15 expression .
	manualset3
216585	2	420003	7	NULL	NULL	0	NULL	 inhibitory effect 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SCP1 overexpression also counteracts the inhibitory effect of epidermal growth factor on TGF-beta-induced p15 expression .
	manualset3
216586	3	420003	7	NULL	NULL	0	NULL	epidermal growth factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	SCP1 overexpression also counteracts the inhibitory effect of epidermal growth factor on TGF-beta-induced p15 expression .
	manualset3
216587	4	420003	7	NULL	NULL	0	NULL	TGF-beta-induced p15 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SCP1 overexpression also counteracts the inhibitory effect of epidermal growth factor on TGF-beta-induced p15 expression .
	manualset3
216588	1	420004	7	NULL	NULL	0	NULL	Myoglobinuria	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Myoglobinuria may result from muscle trauma , ischemia , metabolic causes , drug-induced injury or intrinsic muscle disorders .
	manualset3
216589	2	420004	7	NULL	NULL	0	NULL	muscle trauma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Myoglobinuria may result from muscle trauma , ischemia , metabolic causes , drug-induced injury or intrinsic muscle disorders .
	manualset3
216590	3	420004	7	NULL	NULL	0	NULL	ischemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Myoglobinuria may result from muscle trauma , ischemia , metabolic causes , drug-induced injury or intrinsic muscle disorders .
	manualset3
216591	4	420004	7	NULL	NULL	0	NULL	metabolic causes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Myoglobinuria may result from muscle trauma , ischemia , metabolic causes , drug-induced injury or intrinsic muscle disorders .
	manualset3
216592	5	420004	7	NULL	NULL	0	NULL	drug-induced injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Myoglobinuria may result from muscle trauma , ischemia , metabolic causes , drug-induced injury or intrinsic muscle disorders .
	manualset3
216593	6	420004	7	NULL	NULL	0	NULL	intrinsic muscle disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Myoglobinuria may result from muscle trauma , ischemia , metabolic causes , drug-induced injury or intrinsic muscle disorders .
	manualset3
216594	1	420005	7	NULL	NULL	0	NULL	Twelve point mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve point mutations ( 27 % ) were detected in tumor tissues using single-strand conformation polymorphism analysis followed by direct DNA sequencing .
	manualset3
216595	2	420005	7	NULL	NULL	0	NULL	27 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve point mutations ( 27 % ) were detected in tumor tissues using single-strand conformation polymorphism analysis followed by direct DNA sequencing .
	manualset3
216596	3	420005	7	NULL	NULL	0	NULL	tumor tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve point mutations ( 27 % ) were detected in tumor tissues using single-strand conformation polymorphism analysis followed by direct DNA sequencing .
	manualset3
216597	4	420005	7	NULL	NULL	0	NULL	single-strand conformation polymorphism analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve point mutations ( 27 % ) were detected in tumor tissues using single-strand conformation polymorphism analysis followed by direct DNA sequencing .
	manualset3
216598	5	420005	7	NULL	NULL	0	NULL	direct DNA sequencing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Twelve point mutations ( 27 % ) were detected in tumor tissues using single-strand conformation polymorphism analysis followed by direct DNA sequencing .
	manualset3
216599	1	420006	7	NULL	NULL	0	NULL	mechanisms 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the mechanisms for sustained chemokine gradients and recurring cell infiltration in sterile peritonitis have not been elucidated , toll-like receptors ( TLRs ) have been implicated .
	manualset3
216600	2	420006	7	NULL	NULL	NULL	NULL	sustained chemokine gradients 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although the mechanisms for sustained chemokine gradients and recurring cell infiltration in sterile peritonitis have not been elucidated , toll-like receptors ( TLRs ) have been implicated .
	manualset3
216601	3	420006	7	NULL	NULL	0	NULL	recurring cell infiltration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the mechanisms for sustained chemokine gradients and recurring cell infiltration in sterile peritonitis have not been elucidated , toll-like receptors ( TLRs ) have been implicated .
	manualset3
216602	4	420006	7	NULL	NULL	0	NULL	sterile peritonitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the mechanisms for sustained chemokine gradients and recurring cell infiltration in sterile peritonitis have not been elucidated , toll-like receptors ( TLRs ) have been implicated .
	manualset3
216603	5	420006	7	NULL	NULL	0	NULL	toll-like receptors ( TLRs )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the mechanisms for sustained chemokine gradients and recurring cell infiltration in sterile peritonitis have not been elucidated , toll-like receptors ( TLRs ) have been implicated .
	manualset3
216604	1	420007	7	NULL	NULL	0	NULL	Abstract Objective	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Objective : The purpose of this report is to review key data on the angiotensin receptor blocker ( ARB ) valsartan , along with data from several pivotal studies with other ARBs and angiotensin-converting enzyme ( ACE ) inhibitors , to highlight the beneficial class effects of renin-angiotensin-aldosterone system ( RAAS ) blockade throughout the renal continuum .
	manualset3
216605	2	420007	7	NULL	NULL	0	NULL	purpose	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Objective : The purpose of this report is to review key data on the angiotensin receptor blocker ( ARB ) valsartan , along with data from several pivotal studies with other ARBs and angiotensin-converting enzyme ( ACE ) inhibitors , to highlight the beneficial class effects of renin-angiotensin-aldosterone system ( RAAS ) blockade throughout the renal continuum .
	manualset3
216606	3	420007	7	NULL	NULL	0	NULL	 report 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Objective : The purpose of this report is to review key data on the angiotensin receptor blocker ( ARB ) valsartan , along with data from several pivotal studies with other ARBs and angiotensin-converting enzyme ( ACE ) inhibitors , to highlight the beneficial class effects of renin-angiotensin-aldosterone system ( RAAS ) blockade throughout the renal continuum .
	manualset3
216607	4	420007	7	NULL	NULL	0	NULL	key data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Objective : The purpose of this report is to review key data on the angiotensin receptor blocker ( ARB ) valsartan , along with data from several pivotal studies with other ARBs and angiotensin-converting enzyme ( ACE ) inhibitors , to highlight the beneficial class effects of renin-angiotensin-aldosterone system ( RAAS ) blockade throughout the renal continuum .
	manualset3
216608	5	420007	7	NULL	NULL	NULL	NULL	angiotensin receptor blocker ( ARB )	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Abstract Objective : The purpose of this report is to review key data on the angiotensin receptor blocker ( ARB ) valsartan , along with data from several pivotal studies with other ARBs and angiotensin-converting enzyme ( ACE ) inhibitors , to highlight the beneficial class effects of renin-angiotensin-aldosterone system ( RAAS ) blockade throughout the renal continuum .
	manualset3
216609	6	420007	7	NULL	NULL	0	NULL	valsartan	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Objective : The purpose of this report is to review key data on the angiotensin receptor blocker ( ARB ) valsartan , along with data from several pivotal studies with other ARBs and angiotensin-converting enzyme ( ACE ) inhibitors , to highlight the beneficial class effects of renin-angiotensin-aldosterone system ( RAAS ) blockade throughout the renal continuum .
	manualset3
216610	7	420007	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Objective : The purpose of this report is to review key data on the angiotensin receptor blocker ( ARB ) valsartan , along with data from several pivotal studies with other ARBs and angiotensin-converting enzyme ( ACE ) inhibitors , to highlight the beneficial class effects of renin-angiotensin-aldosterone system ( RAAS ) blockade throughout the renal continuum .
	manualset3
216611	8	420007	7	NULL	NULL	0	NULL	several pivotal studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Objective : The purpose of this report is to review key data on the angiotensin receptor blocker ( ARB ) valsartan , along with data from several pivotal studies with other ARBs and angiotensin-converting enzyme ( ACE ) inhibitors , to highlight the beneficial class effects of renin-angiotensin-aldosterone system ( RAAS ) blockade throughout the renal continuum .
	manualset3
216612	9	420007	7	NULL	NULL	0	NULL	ARBs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Objective : The purpose of this report is to review key data on the angiotensin receptor blocker ( ARB ) valsartan , along with data from several pivotal studies with other ARBs and angiotensin-converting enzyme ( ACE ) inhibitors , to highlight the beneficial class effects of renin-angiotensin-aldosterone system ( RAAS ) blockade throughout the renal continuum .
	manualset3
216613	10	420007	7	NULL	NULL	0	NULL	angiotensin-converting enzyme ( ACE ) inhibitors	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Objective : The purpose of this report is to review key data on the angiotensin receptor blocker ( ARB ) valsartan , along with data from several pivotal studies with other ARBs and angiotensin-converting enzyme ( ACE ) inhibitors , to highlight the beneficial class effects of renin-angiotensin-aldosterone system ( RAAS ) blockade throughout the renal continuum .
	manualset3
216614	11	420007	7	NULL	NULL	0	NULL	 beneficial class effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Objective : The purpose of this report is to review key data on the angiotensin receptor blocker ( ARB ) valsartan , along with data from several pivotal studies with other ARBs and angiotensin-converting enzyme ( ACE ) inhibitors , to highlight the beneficial class effects of renin-angiotensin-aldosterone system ( RAAS ) blockade throughout the renal continuum .
	manualset3
216615	12	420007	7	NULL	NULL	0	NULL	renin-angiotensin-aldosterone system ( RAAS )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Objective : The purpose of this report is to review key data on the angiotensin receptor blocker ( ARB ) valsartan , along with data from several pivotal studies with other ARBs and angiotensin-converting enzyme ( ACE ) inhibitors , to highlight the beneficial class effects of renin-angiotensin-aldosterone system ( RAAS ) blockade throughout the renal continuum .
	manualset3
216616	13	420007	7	NULL	NULL	0	NULL	renal continuum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Objective : The purpose of this report is to review key data on the angiotensin receptor blocker ( ARB ) valsartan , along with data from several pivotal studies with other ARBs and angiotensin-converting enzyme ( ACE ) inhibitors , to highlight the beneficial class effects of renin-angiotensin-aldosterone system ( RAAS ) blockade throughout the renal continuum .
	manualset3
216617	1	420008	7	NULL	NULL	0	NULL	Latency-associated transcript ( LAT ) deletion mutants	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Latency-associated transcript ( LAT ) deletion mutants of herpes simplex virus type 1 ( HSV-1 ) have reduced reactivation phenotypes .
	manualset3
216618	2	420008	7	NULL	NULL	0	NULL	herpes simplex virus type 1 ( HSV-1 )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Latency-associated transcript ( LAT ) deletion mutants of herpes simplex virus type 1 ( HSV-1 ) have reduced reactivation phenotypes .
	manualset3
216619	3	420008	7	NULL	NULL	0	NULL	reactivation phenotypes 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Latency-associated transcript ( LAT ) deletion mutants of herpes simplex virus type 1 ( HSV-1 ) have reduced reactivation phenotypes .
	manualset3
216620	1	420009	7	NULL	NULL	0	NULL	overall success rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An overall success rate of 96.8 per cent was achieved ; and this agent and method warrant further clinical evaluation .
	manualset3
216621	2	420009	7	NULL	NULL	0	NULL	96.8 per cent	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An overall success rate of 96.8 per cent was achieved ; and this agent and method warrant further clinical evaluation .
	manualset3
216622	3	420009	7	NULL	NULL	0	NULL	agent 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	An overall success rate of 96.8 per cent was achieved ; and this agent and method warrant further clinical evaluation .
	manualset3
216623	4	420009	7	NULL	NULL	0	NULL	method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	An overall success rate of 96.8 per cent was achieved ; and this agent and method warrant further clinical evaluation .
	manualset3
216624	5	420009	7	NULL	NULL	0	NULL	clinical evaluation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An overall success rate of 96.8 per cent was achieved ; and this agent and method warrant further clinical evaluation .
	manualset3
216625	1	420010	7	NULL	NULL	0	NULL	Ambulatory treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ambulatory treatment of phlebitis with enzyme tablets .
	manualset3
216626	2	420010	7	NULL	NULL	0	NULL	phlebitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Ambulatory treatment of phlebitis with enzyme tablets .
	manualset3
216627	3	420010	7	NULL	NULL	0	NULL	enzyme tablets	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Ambulatory treatment of phlebitis with enzyme tablets .
	manualset3
216628	1	420011	7	NULL	NULL	0	NULL	 fourth generation	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Toward a fourth generation of health planning .
	manualset3
216629	2	420011	7	NULL	NULL	0	NULL	health planning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Toward a fourth generation of health planning .
	manualset3
216630	1	420012	7	NULL	NULL	NULL	NULL	natural head position	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During natural head position , only the activity of sternocleidomastoid muscle on the natural tilting side was increased .
	manualset3
216631	2	420012	7	NULL	NULL	0	NULL	activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	During natural head position , only the activity of sternocleidomastoid muscle on the natural tilting side was increased .
	manualset3
216632	3	420012	7	NULL	NULL	0	NULL	sternocleidomastoid muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	During natural head position , only the activity of sternocleidomastoid muscle on the natural tilting side was increased .
	manualset3
216633	4	420012	7	NULL	NULL	0	NULL	natural tilting side	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	During natural head position , only the activity of sternocleidomastoid muscle on the natural tilting side was increased .
	manualset3
216634	1	420013	7	NULL	NULL	0	NULL	morphometric correlation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , there is usually , but not always a morphometric correlation of the severity of changes between peripheral nerves and muscle .
	manualset3
216635	2	420013	7	NULL	NULL	0	NULL	severity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , there is usually , but not always a morphometric correlation of the severity of changes between peripheral nerves and muscle .
	manualset3
216636	3	420013	7	NULL	NULL	0	NULL	changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , there is usually , but not always a morphometric correlation of the severity of changes between peripheral nerves and muscle .
	manualset3
216637	4	420013	7	NULL	NULL	0	NULL	peripheral nerves	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , there is usually , but not always a morphometric correlation of the severity of changes between peripheral nerves and muscle .
	manualset3
216638	5	420013	7	NULL	NULL	0	NULL	muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , there is usually , but not always a morphometric correlation of the severity of changes between peripheral nerves and muscle .
	manualset3
216639	1	420014	7	NULL	NULL	0	NULL	 problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The problems for their effective application are fundamentally delivery , stability and off-target effects .
	manualset3
216640	2	420014	7	NULL	NULL	0	NULL	effective application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The problems for their effective application are fundamentally delivery , stability and off-target effects .
	manualset3
216641	3	420014	7	NULL	NULL	0	NULL	delivery 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The problems for their effective application are fundamentally delivery , stability and off-target effects .
	manualset3
216642	4	420014	7	NULL	NULL	0	NULL	stability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The problems for their effective application are fundamentally delivery , stability and off-target effects .
	manualset3
216643	5	420014	7	NULL	NULL	0	NULL	off-target effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The problems for their effective application are fundamentally delivery , stability and off-target effects .
	manualset3
216644	1	420015	7	NULL	NULL	0	NULL	morphological characteristics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the morphological characteristics of the lesion seemed easy to pass through the obstruction with the guide wire , the balloon dilatation was not possible because of the hardness of a chronic lesion lasting that long .
	manualset3
216645	2	420015	7	NULL	NULL	0	NULL	lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the morphological characteristics of the lesion seemed easy to pass through the obstruction with the guide wire , the balloon dilatation was not possible because of the hardness of a chronic lesion lasting that long .
	manualset3
216646	3	420015	7	NULL	NULL	0	NULL	obstruction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the morphological characteristics of the lesion seemed easy to pass through the obstruction with the guide wire , the balloon dilatation was not possible because of the hardness of a chronic lesion lasting that long .
	manualset3
216647	4	420015	7	NULL	NULL	0	NULL	guide wire	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the morphological characteristics of the lesion seemed easy to pass through the obstruction with the guide wire , the balloon dilatation was not possible because of the hardness of a chronic lesion lasting that long .
	manualset3
216648	5	420015	7	NULL	NULL	0	NULL	balloon dilatation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the morphological characteristics of the lesion seemed easy to pass through the obstruction with the guide wire , the balloon dilatation was not possible because of the hardness of a chronic lesion lasting that long .
	manualset3
216649	6	420015	7	NULL	NULL	0	NULL	hardness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the morphological characteristics of the lesion seemed easy to pass through the obstruction with the guide wire , the balloon dilatation was not possible because of the hardness of a chronic lesion lasting that long .
	manualset3
216650	7	420015	7	NULL	NULL	0	NULL	chronic lesion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the morphological characteristics of the lesion seemed easy to pass through the obstruction with the guide wire , the balloon dilatation was not possible because of the hardness of a chronic lesion lasting that long .
	manualset3
216651	1	420016	7	NULL	NULL	0	NULL	Enzymatic asymmetric synthesis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Enzymatic asymmetric synthesis by decarboxylases .
	manualset3
216652	2	420016	7	NULL	NULL	0	NULL	decarboxylases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Enzymatic asymmetric synthesis by decarboxylases .
	manualset3
216653	1	420017	7	NULL	NULL	0	NULL	 effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of RU24969 ( 1 and 5 microM ) was prevented by concurrent infusion of methiothepin ( 1 and 10 microM ) into the anterior hypothalamus via the microdialysis probe .
	manualset3
216654	2	420017	7	NULL	NULL	0	NULL	RU24969	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of RU24969 ( 1 and 5 microM ) was prevented by concurrent infusion of methiothepin ( 1 and 10 microM ) into the anterior hypothalamus via the microdialysis probe .
	manualset3
216655	3	420017	7	NULL	NULL	0	NULL	1 microM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of RU24969 ( 1 and 5 microM ) was prevented by concurrent infusion of methiothepin ( 1 and 10 microM ) into the anterior hypothalamus via the microdialysis probe .
	manualset3
216656	4	420017	7	NULL	NULL	0	NULL	5 microM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of RU24969 ( 1 and 5 microM ) was prevented by concurrent infusion of methiothepin ( 1 and 10 microM ) into the anterior hypothalamus via the microdialysis probe .
	manualset3
216657	5	420017	7	NULL	NULL	0	NULL	concurrent infusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of RU24969 ( 1 and 5 microM ) was prevented by concurrent infusion of methiothepin ( 1 and 10 microM ) into the anterior hypothalamus via the microdialysis probe .
	manualset3
216658	6	420017	7	NULL	NULL	0	NULL	methiothepin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of RU24969 ( 1 and 5 microM ) was prevented by concurrent infusion of methiothepin ( 1 and 10 microM ) into the anterior hypothalamus via the microdialysis probe .
	manualset3
216659	7	420017	7	NULL	NULL	0	NULL	1 microM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of RU24969 ( 1 and 5 microM ) was prevented by concurrent infusion of methiothepin ( 1 and 10 microM ) into the anterior hypothalamus via the microdialysis probe .
	manualset3
216660	8	420017	7	NULL	NULL	0	NULL	10 microM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of RU24969 ( 1 and 5 microM ) was prevented by concurrent infusion of methiothepin ( 1 and 10 microM ) into the anterior hypothalamus via the microdialysis probe .
	manualset3
216661	9	420017	7	NULL	NULL	0	NULL	anterior hypothalamus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of RU24969 ( 1 and 5 microM ) was prevented by concurrent infusion of methiothepin ( 1 and 10 microM ) into the anterior hypothalamus via the microdialysis probe .
	manualset3
216662	10	420017	7	NULL	NULL	0	NULL	microdialysis probe	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of RU24969 ( 1 and 5 microM ) was prevented by concurrent infusion of methiothepin ( 1 and 10 microM ) into the anterior hypothalamus via the microdialysis probe .
	manualset3
216663	1	420018	7	NULL	NULL	0	NULL	DOBV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	DOBV was present in 17.5 % of asymptomatic subjects and , interestingly , the preferential hantavirus serotype could not be determined in 12.7 % of the asymptomatic antibody-positive subjects .
	manualset3
216664	2	420018	7	NULL	NULL	0	NULL	17.5 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	DOBV was present in 17.5 % of asymptomatic subjects and , interestingly , the preferential hantavirus serotype could not be determined in 12.7 % of the asymptomatic antibody-positive subjects .
	manualset3
216665	3	420018	7	NULL	NULL	0	NULL	asymptomatic subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	DOBV was present in 17.5 % of asymptomatic subjects and , interestingly , the preferential hantavirus serotype could not be determined in 12.7 % of the asymptomatic antibody-positive subjects .
	manualset3
216666	4	420018	7	NULL	NULL	0	NULL	 hantavirus serotype	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	DOBV was present in 17.5 % of asymptomatic subjects and , interestingly , the preferential hantavirus serotype could not be determined in 12.7 % of the asymptomatic antibody-positive subjects .
	manualset3
216667	5	420018	7	NULL	NULL	0	NULL	12.7 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	DOBV was present in 17.5 % of asymptomatic subjects and , interestingly , the preferential hantavirus serotype could not be determined in 12.7 % of the asymptomatic antibody-positive subjects .
	manualset3
216668	6	420018	7	NULL	NULL	0	NULL	asymptomatic antibody-positive subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	DOBV was present in 17.5 % of asymptomatic subjects and , interestingly , the preferential hantavirus serotype could not be determined in 12.7 % of the asymptomatic antibody-positive subjects .
	manualset3
216669	1	420019	7	NULL	NULL	0	NULL	notion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This notion is not supported by the biochemistry nor the molecular biology .
	manualset3
216670	2	420019	7	NULL	NULL	0	NULL	biochemistry	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This notion is not supported by the biochemistry nor the molecular biology .
	manualset3
216671	3	420019	7	NULL	NULL	0	NULL	molecular biology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This notion is not supported by the biochemistry nor the molecular biology .
	manualset3
216672	1	420020	7	NULL	NULL	0	NULL	components 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The most prominent of these are components of the thyroid hormone receptor-associated protein ( TRAP ) / Mediator coactivator complex , which interacts with ERalpha and ERbeta in both unfractionated nuclear extracts and purified form .
	manualset3
216673	2	420020	7	NULL	NULL	0	NULL	 thyroid hormone receptor-associated protein ( TRAP ) / Mediator coactivator complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The most prominent of these are components of the thyroid hormone receptor-associated protein ( TRAP ) / Mediator coactivator complex , which interacts with ERalpha and ERbeta in both unfractionated nuclear extracts and purified form .
	manualset3
216674	3	420020	7	NULL	NULL	0	NULL	ERalpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The most prominent of these are components of the thyroid hormone receptor-associated protein ( TRAP ) / Mediator coactivator complex , which interacts with ERalpha and ERbeta in both unfractionated nuclear extracts and purified form .
	manualset3
216675	4	420020	7	NULL	NULL	0	NULL	ERbeta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The most prominent of these are components of the thyroid hormone receptor-associated protein ( TRAP ) / Mediator coactivator complex , which interacts with ERalpha and ERbeta in both unfractionated nuclear extracts and purified form .
	manualset3
216676	5	420020	7	NULL	NULL	0	NULL	unfractionated nuclear extracts 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The most prominent of these are components of the thyroid hormone receptor-associated protein ( TRAP ) / Mediator coactivator complex , which interacts with ERalpha and ERbeta in both unfractionated nuclear extracts and purified form .
	manualset3
217442	6	420020	7	NULL	NULL	NULL	NULL	purified form	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The most prominent of these are components of the thyroid hormone receptor-associated protein ( TRAP ) / Mediator coactivator complex , which interacts with ERalpha and ERbeta in both unfractionated nuclear extracts and purified form .
	manualset3
216677	1	420021	7	NULL	NULL	0	NULL	series	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of monoclonal antibodies ( mAbs ) against human CETP was obtained , comprising mAbs either inhibiting or not inhibiting these transfer activities .
	manualset3
216678	2	420021	7	NULL	NULL	0	NULL	monoclonal antibodies ( mAbs )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of monoclonal antibodies ( mAbs ) against human CETP was obtained , comprising mAbs either inhibiting or not inhibiting these transfer activities .
	manualset3
216679	3	420021	7	NULL	NULL	0	NULL	human CETP 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of monoclonal antibodies ( mAbs ) against human CETP was obtained , comprising mAbs either inhibiting or not inhibiting these transfer activities .
	manualset3
216680	4	420021	7	NULL	NULL	0	NULL	mAbs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of monoclonal antibodies ( mAbs ) against human CETP was obtained , comprising mAbs either inhibiting or not inhibiting these transfer activities .
	manualset3
216681	5	420021	7	NULL	NULL	0	NULL	transfer activities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A series of monoclonal antibodies ( mAbs ) against human CETP was obtained , comprising mAbs either inhibiting or not inhibiting these transfer activities .
	manualset3
216682	1	420022	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A study was considered positive when ventricular tachycardia , defined as 10 or more consecutive ventricular beats , was induced by any pacing modality .
	manualset3
216683	2	420022	7	NULL	NULL	0	NULL	ventricular tachycardia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A study was considered positive when ventricular tachycardia , defined as 10 or more consecutive ventricular beats , was induced by any pacing modality .
	manualset3
216684	3	420022	7	NULL	NULL	0	NULL	 10	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A study was considered positive when ventricular tachycardia , defined as 10 or more consecutive ventricular beats , was induced by any pacing modality .
	manualset3
216685	4	420022	7	NULL	NULL	0	NULL	ventricular beats 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A study was considered positive when ventricular tachycardia , defined as 10 or more consecutive ventricular beats , was induced by any pacing modality .
	manualset3
216686	5	420022	7	NULL	NULL	0	NULL	pacing modality	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A study was considered positive when ventricular tachycardia , defined as 10 or more consecutive ventricular beats , was induced by any pacing modality .
	manualset3
216687	1	420023	7	NULL	NULL	0	NULL	Biosynthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Biosynthesis of GlyCAM-1 , a mucin-like ligand for L-selectin .
	manualset3
216688	2	420023	7	NULL	NULL	0	NULL	GlyCAM-1	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Biosynthesis of GlyCAM-1 , a mucin-like ligand for L-selectin .
	manualset3
216689	3	420023	7	NULL	NULL	0	NULL	mucin-like ligand	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Biosynthesis of GlyCAM-1 , a mucin-like ligand for L-selectin .
	manualset3
216690	4	420023	7	NULL	NULL	0	NULL	L-selectin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Biosynthesis of GlyCAM-1 , a mucin-like ligand for L-selectin .
	manualset3
216691	1	420024	7	NULL	NULL	0	NULL	preparations 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolated and carefully purified preparations of the sarcolemmal membrane from rat cardiac muscle were used to study the membrane-bound protein kinase ( PrK ) reaction .
	manualset3
216692	2	420024	7	NULL	NULL	0	NULL	sarcolemmal membrane	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolated and carefully purified preparations of the sarcolemmal membrane from rat cardiac muscle were used to study the membrane-bound protein kinase ( PrK ) reaction .
	manualset3
216693	3	420024	7	NULL	NULL	0	NULL	 rat cardiac muscle 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolated and carefully purified preparations of the sarcolemmal membrane from rat cardiac muscle were used to study the membrane-bound protein kinase ( PrK ) reaction .
	manualset3
216694	4	420024	7	NULL	NULL	0	NULL	membrane-bound protein kinase ( PrK ) reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolated and carefully purified preparations of the sarcolemmal membrane from rat cardiac muscle were used to study the membrane-bound protein kinase ( PrK ) reaction .
	manualset3
216695	1	420025	7	NULL	NULL	0	NULL	Ca ( 2 + ) - activated Cl ( - ) current 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Ca ( 2 + ) - activated Cl ( - ) current in rabbit sinoatrial node cells .
	manualset3
216696	2	420025	7	NULL	NULL	0	NULL	rabbit sinoatrial node cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Ca ( 2 + ) - activated Cl ( - ) current in rabbit sinoatrial node cells .
	manualset3
216697	1	420026	7	NULL	NULL	0	NULL	negligible sample volumes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The negligible sample volumes used in the microchip procedure obviates surface fouling common to amperometric measurements of phenolic compounds .
	manualset3
216698	2	420026	7	NULL	NULL	0	NULL	microchip procedure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The negligible sample volumes used in the microchip procedure obviates surface fouling common to amperometric measurements of phenolic compounds .
	manualset3
216699	3	420026	7	NULL	NULL	0	NULL	surface fouling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The negligible sample volumes used in the microchip procedure obviates surface fouling common to amperometric measurements of phenolic compounds .
	manualset3
216700	4	420026	7	NULL	NULL	0	NULL	amperometric measurements	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The negligible sample volumes used in the microchip procedure obviates surface fouling common to amperometric measurements of phenolic compounds .
	manualset3
216701	5	420026	7	NULL	NULL	0	NULL	phenolic compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The negligible sample volumes used in the microchip procedure obviates surface fouling common to amperometric measurements of phenolic compounds .
	manualset3
216702	1	420027	7	NULL	NULL	0	NULL	haloperidol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Determination of haloperidol and reduced haloperidol in the plasma and blood of patients on depot haloperidol .
	manualset3
216703	2	420027	7	NULL	NULL	0	NULL	haloperidol 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Determination of haloperidol and reduced haloperidol in the plasma and blood of patients on depot haloperidol .
	manualset3
216704	3	420027	7	NULL	NULL	0	NULL	plasma 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Determination of haloperidol and reduced haloperidol in the plasma and blood of patients on depot haloperidol .
	manualset3
216705	4	420027	7	NULL	NULL	0	NULL	blood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Determination of haloperidol and reduced haloperidol in the plasma and blood of patients on depot haloperidol .
	manualset3
216706	5	420027	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Determination of haloperidol and reduced haloperidol in the plasma and blood of patients on depot haloperidol .
	manualset3
216707	6	420027	7	NULL	NULL	0	NULL	depot haloperidol 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Determination of haloperidol and reduced haloperidol in the plasma and blood of patients on depot haloperidol .
	manualset3
217443	7	420027	7	NULL	NULL	0	NULL	Determination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Determination of haloperidol and reduced haloperidol in the plasma and blood of patients on depot haloperidol .
	manualset3
216708	1	420028	7	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , treatment of HIV with either chemical agents or strong acids will effectively inactivate the AIDS virus .
	manualset3
216709	2	420028	7	NULL	NULL	0	NULL	HIV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , treatment of HIV with either chemical agents or strong acids will effectively inactivate the AIDS virus .
	manualset3
216710	3	420028	7	NULL	NULL	0	NULL	chemical agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , treatment of HIV with either chemical agents or strong acids will effectively inactivate the AIDS virus .
	manualset3
216711	4	420028	7	NULL	NULL	0	NULL	strong acids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , treatment of HIV with either chemical agents or strong acids will effectively inactivate the AIDS virus .
	manualset3
216712	5	420028	7	NULL	NULL	0	NULL	AIDS virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , treatment of HIV with either chemical agents or strong acids will effectively inactivate the AIDS virus .
	manualset3
216713	1	420029	7	NULL	NULL	NULL	NULL	Part 1	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Part 1 : cytotoxicity to corneal endothelial cells in a rabbit model .
	manualset3
216714	2	420029	7	NULL	NULL	0	NULL	cytotoxicity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Part 1 : cytotoxicity to corneal endothelial cells in a rabbit model .
	manualset3
216715	3	420029	7	NULL	NULL	0	NULL	corneal endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Part 1 : cytotoxicity to corneal endothelial cells in a rabbit model .
	manualset3
216716	4	420029	7	NULL	NULL	0	NULL	rabbit model 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Part 1 : cytotoxicity to corneal endothelial cells in a rabbit model .
	manualset3
216717	1	420030	7	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data are consistent with a transition state in which the charge on the aldehyde carbonyl increases relative to the charge on this group in the ground state .
	manualset3
216718	2	420030	7	NULL	NULL	0	NULL	transition state	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data are consistent with a transition state in which the charge on the aldehyde carbonyl increases relative to the charge on this group in the ground state .
	manualset3
216719	3	420030	7	NULL	NULL	0	NULL	charge	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data are consistent with a transition state in which the charge on the aldehyde carbonyl increases relative to the charge on this group in the ground state .
	manualset3
216720	4	420030	7	NULL	NULL	0	NULL	aldehyde carbonyl 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data are consistent with a transition state in which the charge on the aldehyde carbonyl increases relative to the charge on this group in the ground state .
	manualset3
216721	5	420030	7	NULL	NULL	0	NULL	charge	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data are consistent with a transition state in which the charge on the aldehyde carbonyl increases relative to the charge on this group in the ground state .
	manualset3
216722	6	420030	7	NULL	NULL	0	NULL	group	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data are consistent with a transition state in which the charge on the aldehyde carbonyl increases relative to the charge on this group in the ground state .
	manualset3
216723	7	420030	7	NULL	NULL	0	NULL	ground state	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These data are consistent with a transition state in which the charge on the aldehyde carbonyl increases relative to the charge on this group in the ground state .
	manualset3
216726	1	420031	7	NULL	NULL	0	NULL	comparison	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of free and bound sNRE shows that the NRE loop becomes structured upon binding .
	manualset3
216727	2	420031	7	NULL	NULL	0	NULL	free sNRE	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of free and bound sNRE shows that the NRE loop becomes structured upon binding .
	manualset3
216728	3	420031	7	NULL	NULL	0	NULL	bound sNRE	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of free and bound sNRE shows that the NRE loop becomes structured upon binding .
	manualset3
216729	4	420031	7	NULL	NULL	0	NULL	NRE loop	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of free and bound sNRE shows that the NRE loop becomes structured upon binding .
	manualset3
216730	5	420031	7	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of free and bound sNRE shows that the NRE loop becomes structured upon binding .
	manualset3
216731	1	420032	7	NULL	NULL	0	NULL	discovery	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the discovery of the TRP channel superfamily and their involvement in receptor-induced Ca ( 2 + ) entry , many studies have shown that different members of the TRP superfamily translocate into the plasma membrane upon stimulation .
	manualset3
216732	2	420032	7	NULL	NULL	0	NULL	TRP channel superfamily	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the discovery of the TRP channel superfamily and their involvement in receptor-induced Ca ( 2 + ) entry , many studies have shown that different members of the TRP superfamily translocate into the plasma membrane upon stimulation .
	manualset3
216733	3	420032	7	NULL	NULL	0	NULL	receptor-induced Ca ( 2 + ) entry	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the discovery of the TRP channel superfamily and their involvement in receptor-induced Ca ( 2 + ) entry , many studies have shown that different members of the TRP superfamily translocate into the plasma membrane upon stimulation .
	manualset3
216734	4	420032	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the discovery of the TRP channel superfamily and their involvement in receptor-induced Ca ( 2 + ) entry , many studies have shown that different members of the TRP superfamily translocate into the plasma membrane upon stimulation .
	manualset3
216735	5	420032	7	NULL	NULL	0	NULL	different members	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the discovery of the TRP channel superfamily and their involvement in receptor-induced Ca ( 2 + ) entry , many studies have shown that different members of the TRP superfamily translocate into the plasma membrane upon stimulation .
	manualset3
216736	6	420032	7	NULL	NULL	0	NULL	TRP superfamily 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the discovery of the TRP channel superfamily and their involvement in receptor-induced Ca ( 2 + ) entry , many studies have shown that different members of the TRP superfamily translocate into the plasma membrane upon stimulation .
	manualset3
216737	7	420032	7	NULL	NULL	0	NULL	plasma membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the discovery of the TRP channel superfamily and their involvement in receptor-induced Ca ( 2 + ) entry , many studies have shown that different members of the TRP superfamily translocate into the plasma membrane upon stimulation .
	manualset3
216738	8	420032	7	NULL	NULL	0	NULL	stimulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the discovery of the TRP channel superfamily and their involvement in receptor-induced Ca ( 2 + ) entry , many studies have shown that different members of the TRP superfamily translocate into the plasma membrane upon stimulation .
	manualset3
218214	9	420032	7	NULL	NULL	0	NULL	involvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the discovery of the TRP channel superfamily and their involvement in receptor-induced Ca ( 2 + ) entry , many studies have shown that different members of the TRP superfamily translocate into the plasma membrane upon stimulation .
	manualset3
216739	1	420033	7	NULL	NULL	0	NULL	size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The size of the macrometastases became larger , and the frequency of micrometastases and the distance of micrometastases from macrometastases had a tendency to increase .
	manualset3
216740	2	420033	7	NULL	NULL	0	NULL	macrometastases	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The size of the macrometastases became larger , and the frequency of micrometastases and the distance of micrometastases from macrometastases had a tendency to increase .
	manualset3
216741	3	420033	7	NULL	NULL	0	NULL	frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The size of the macrometastases became larger , and the frequency of micrometastases and the distance of micrometastases from macrometastases had a tendency to increase .
	manualset3
216742	4	420033	7	NULL	NULL	0	NULL	micrometastases	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The size of the macrometastases became larger , and the frequency of micrometastases and the distance of micrometastases from macrometastases had a tendency to increase .
	manualset3
216743	5	420033	7	NULL	NULL	0	NULL	distance	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The size of the macrometastases became larger , and the frequency of micrometastases and the distance of micrometastases from macrometastases had a tendency to increase .
	manualset3
216744	6	420033	7	NULL	NULL	0	NULL	micrometastases	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The size of the macrometastases became larger , and the frequency of micrometastases and the distance of micrometastases from macrometastases had a tendency to increase .
	manualset3
216745	7	420033	7	NULL	NULL	0	NULL	macrometastases	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The size of the macrometastases became larger , and the frequency of micrometastases and the distance of micrometastases from macrometastases had a tendency to increase .
	manualset3
216746	1	420034	7	NULL	NULL	0	NULL	Uhysiological DDD	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Uhysiological DDD or QT pacing .
	manualset3
216747	2	420034	7	NULL	NULL	0	NULL	QT pacing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Uhysiological DDD or QT pacing .
	manualset3
216748	1	420035	7	NULL	NULL	0	NULL	Vascular sinus transformation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Vascular sinus transformation of the lymph nodes .
	manualset3
216749	2	420035	7	NULL	NULL	0	NULL	lymph nodes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Vascular sinus transformation of the lymph nodes .
	manualset3
216750	1	420036	7	NULL	NULL	0	NULL	lipid oxidation rate	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The lipid oxidation rate was decreased ( 0.63 + / - 0.05 versus 1.02 + / - 0.08 mg min-1 kg-1 , P less than 0.001 ) , whereas there was a significant increase in the carbohydrate oxidation rate ( 1.93 + / - 0.17 versus 1.22 + / - 0.18 mg min-1 kg-1 , P = 0.02 ) .
	manualset3
216751	2	420036	7	NULL	NULL	0	NULL	 0.63 + / - 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The lipid oxidation rate was decreased ( 0.63 + / - 0.05 versus 1.02 + / - 0.08 mg min-1 kg-1 , P less than 0.001 ) , whereas there was a significant increase in the carbohydrate oxidation rate ( 1.93 + / - 0.17 versus 1.22 + / - 0.18 mg min-1 kg-1 , P = 0.02 ) .
	manualset3
216752	3	420036	7	NULL	NULL	0	NULL	1.02 + / - 0.08 mg min-1 kg-1 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The lipid oxidation rate was decreased ( 0.63 + / - 0.05 versus 1.02 + / - 0.08 mg min-1 kg-1 , P less than 0.001 ) , whereas there was a significant increase in the carbohydrate oxidation rate ( 1.93 + / - 0.17 versus 1.22 + / - 0.18 mg min-1 kg-1 , P = 0.02 ) .
	manualset3
216753	4	420036	7	NULL	NULL	0	NULL	P less than 0.001	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The lipid oxidation rate was decreased ( 0.63 + / - 0.05 versus 1.02 + / - 0.08 mg min-1 kg-1 , P less than 0.001 ) , whereas there was a significant increase in the carbohydrate oxidation rate ( 1.93 + / - 0.17 versus 1.22 + / - 0.18 mg min-1 kg-1 , P = 0.02 ) .
	manualset3
216754	5	420036	7	NULL	NULL	0	NULL	 increase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The lipid oxidation rate was decreased ( 0.63 + / - 0.05 versus 1.02 + / - 0.08 mg min-1 kg-1 , P less than 0.001 ) , whereas there was a significant increase in the carbohydrate oxidation rate ( 1.93 + / - 0.17 versus 1.22 + / - 0.18 mg min-1 kg-1 , P = 0.02 ) .
	manualset3
216755	6	420036	7	NULL	NULL	0	NULL	carbohydrate oxidation rate	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The lipid oxidation rate was decreased ( 0.63 + / - 0.05 versus 1.02 + / - 0.08 mg min-1 kg-1 , P less than 0.001 ) , whereas there was a significant increase in the carbohydrate oxidation rate ( 1.93 + / - 0.17 versus 1.22 + / - 0.18 mg min-1 kg-1 , P = 0.02 ) .
	manualset3
216756	7	420036	7	NULL	NULL	0	NULL	1.93 + / - 0.17	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The lipid oxidation rate was decreased ( 0.63 + / - 0.05 versus 1.02 + / - 0.08 mg min-1 kg-1 , P less than 0.001 ) , whereas there was a significant increase in the carbohydrate oxidation rate ( 1.93 + / - 0.17 versus 1.22 + / - 0.18 mg min-1 kg-1 , P = 0.02 ) .
	manualset3
216757	8	420036	7	NULL	NULL	0	NULL	1.22 + / - 0.18 mg min-1 kg-1	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The lipid oxidation rate was decreased ( 0.63 + / - 0.05 versus 1.02 + / - 0.08 mg min-1 kg-1 , P less than 0.001 ) , whereas there was a significant increase in the carbohydrate oxidation rate ( 1.93 + / - 0.17 versus 1.22 + / - 0.18 mg min-1 kg-1 , P = 0.02 ) .
	manualset3
216758	9	420036	7	NULL	NULL	0	NULL	P = 0.02 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The lipid oxidation rate was decreased ( 0.63 + / - 0.05 versus 1.02 + / - 0.08 mg min-1 kg-1 , P less than 0.001 ) , whereas there was a significant increase in the carbohydrate oxidation rate ( 1.93 + / - 0.17 versus 1.22 + / - 0.18 mg min-1 kg-1 , P = 0.02 ) .
	manualset3
216759	1	420037	7	NULL	NULL	0	NULL	Light -microscopic studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Light - and electron-microscopic studies of tumor morphology were combined with biochemical measurements of testosterone , dihydrotestosterone , estrone , estradiol , and progesterone .
	manualset3
216760	2	420037	7	NULL	NULL	0	NULL	 electron-microscopic studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Light - and electron-microscopic studies of tumor morphology were combined with biochemical measurements of testosterone , dihydrotestosterone , estrone , estradiol , and progesterone .
	manualset3
216761	3	420037	7	NULL	NULL	0	NULL	tumor morphology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Light - and electron-microscopic studies of tumor morphology were combined with biochemical measurements of testosterone , dihydrotestosterone , estrone , estradiol , and progesterone .
	manualset3
216762	4	420037	7	NULL	NULL	0	NULL	 biochemical measurements	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Light - and electron-microscopic studies of tumor morphology were combined with biochemical measurements of testosterone , dihydrotestosterone , estrone , estradiol , and progesterone .
	manualset3
216763	5	420037	7	NULL	NULL	0	NULL	testosterone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Light - and electron-microscopic studies of tumor morphology were combined with biochemical measurements of testosterone , dihydrotestosterone , estrone , estradiol , and progesterone .
	manualset3
216764	6	420037	7	NULL	NULL	0	NULL	dihydrotestosterone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Light - and electron-microscopic studies of tumor morphology were combined with biochemical measurements of testosterone , dihydrotestosterone , estrone , estradiol , and progesterone .
	manualset3
216765	7	420037	7	NULL	NULL	0	NULL	estrone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Light - and electron-microscopic studies of tumor morphology were combined with biochemical measurements of testosterone , dihydrotestosterone , estrone , estradiol , and progesterone .
	manualset3
216766	8	420037	7	NULL	NULL	0	NULL	estradiol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Light - and electron-microscopic studies of tumor morphology were combined with biochemical measurements of testosterone , dihydrotestosterone , estrone , estradiol , and progesterone .
	manualset3
216767	9	420037	7	NULL	NULL	0	NULL	progesterone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Light - and electron-microscopic studies of tumor morphology were combined with biochemical measurements of testosterone , dihydrotestosterone , estrone , estradiol , and progesterone .
	manualset3
216768	1	420038	7	NULL	NULL	0	NULL	Multifactorial analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multifactorial analysis of blood pressure level in Allahabad urban community .
	manualset3
216769	2	420038	7	NULL	NULL	0	NULL	blood pressure level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multifactorial analysis of blood pressure level in Allahabad urban community .
	manualset3
216770	3	420038	7	NULL	NULL	0	NULL	Allahabad urban community	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Multifactorial analysis of blood pressure level in Allahabad urban community .
	manualset3
216771	1	420039	7	NULL	NULL	0	NULL	paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper describes the background and evaluates the effectiveness of a flashing green phase just before the amber leading to red phase in the traffic signal cycle .
	manualset3
216772	2	420039	7	NULL	NULL	0	NULL	background	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper describes the background and evaluates the effectiveness of a flashing green phase just before the amber leading to red phase in the traffic signal cycle .
	manualset3
216773	3	420039	7	NULL	NULL	0	NULL	effectiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper describes the background and evaluates the effectiveness of a flashing green phase just before the amber leading to red phase in the traffic signal cycle .
	manualset3
216774	4	420039	7	NULL	NULL	0	NULL	flashing green phase	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper describes the background and evaluates the effectiveness of a flashing green phase just before the amber leading to red phase in the traffic signal cycle .
	manualset3
216775	5	420039	7	NULL	NULL	0	NULL	amber	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper describes the background and evaluates the effectiveness of a flashing green phase just before the amber leading to red phase in the traffic signal cycle .
	manualset3
216776	6	420039	7	NULL	NULL	0	NULL	red phase	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper describes the background and evaluates the effectiveness of a flashing green phase just before the amber leading to red phase in the traffic signal cycle .
	manualset3
216777	7	420039	7	NULL	NULL	0	NULL	traffic signal cycle	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper describes the background and evaluates the effectiveness of a flashing green phase just before the amber leading to red phase in the traffic signal cycle .
	manualset3
216778	1	420040	7	NULL	NULL	0	NULL	 presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of 0.1 mM arachidonic acid , the rate of the reduction of nitroblue tetrazolium ( NBT ) to nitroblue formazan ( NBF ) was stimulated from 0.65 + / - 0.10 to 1.43 + / - 0.15 and from 0.092 + / - 0.006 to 0.162 + / - 0.009 nmol/min/mg protein in intact and broken cell preparations , respectively .
	manualset3
216779	2	420040	7	NULL	NULL	0	NULL	0.1 mM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of 0.1 mM arachidonic acid , the rate of the reduction of nitroblue tetrazolium ( NBT ) to nitroblue formazan ( NBF ) was stimulated from 0.65 + / - 0.10 to 1.43 + / - 0.15 and from 0.092 + / - 0.006 to 0.162 + / - 0.009 nmol/min/mg protein in intact and broken cell preparations , respectively .
	manualset3
216780	3	420040	7	NULL	NULL	0	NULL	arachidonic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of 0.1 mM arachidonic acid , the rate of the reduction of nitroblue tetrazolium ( NBT ) to nitroblue formazan ( NBF ) was stimulated from 0.65 + / - 0.10 to 1.43 + / - 0.15 and from 0.092 + / - 0.006 to 0.162 + / - 0.009 nmol/min/mg protein in intact and broken cell preparations , respectively .
	manualset3
216781	4	420040	7	NULL	NULL	0	NULL	rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of 0.1 mM arachidonic acid , the rate of the reduction of nitroblue tetrazolium ( NBT ) to nitroblue formazan ( NBF ) was stimulated from 0.65 + / - 0.10 to 1.43 + / - 0.15 and from 0.092 + / - 0.006 to 0.162 + / - 0.009 nmol/min/mg protein in intact and broken cell preparations , respectively .
	manualset3
216782	5	420040	7	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of 0.1 mM arachidonic acid , the rate of the reduction of nitroblue tetrazolium ( NBT ) to nitroblue formazan ( NBF ) was stimulated from 0.65 + / - 0.10 to 1.43 + / - 0.15 and from 0.092 + / - 0.006 to 0.162 + / - 0.009 nmol/min/mg protein in intact and broken cell preparations , respectively .
	manualset3
216783	6	420040	7	NULL	NULL	0	NULL	nitroblue tetrazolium ( NBT )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of 0.1 mM arachidonic acid , the rate of the reduction of nitroblue tetrazolium ( NBT ) to nitroblue formazan ( NBF ) was stimulated from 0.65 + / - 0.10 to 1.43 + / - 0.15 and from 0.092 + / - 0.006 to 0.162 + / - 0.009 nmol/min/mg protein in intact and broken cell preparations , respectively .
	manualset3
216784	7	420040	7	NULL	NULL	0	NULL	nitroblue formazan ( NBF )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of 0.1 mM arachidonic acid , the rate of the reduction of nitroblue tetrazolium ( NBT ) to nitroblue formazan ( NBF ) was stimulated from 0.65 + / - 0.10 to 1.43 + / - 0.15 and from 0.092 + / - 0.006 to 0.162 + / - 0.009 nmol/min/mg protein in intact and broken cell preparations , respectively .
	manualset3
216785	8	420040	7	NULL	NULL	0	NULL	0.65 + / - 0.10	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of 0.1 mM arachidonic acid , the rate of the reduction of nitroblue tetrazolium ( NBT ) to nitroblue formazan ( NBF ) was stimulated from 0.65 + / - 0.10 to 1.43 + / - 0.15 and from 0.092 + / - 0.006 to 0.162 + / - 0.009 nmol/min/mg protein in intact and broken cell preparations , respectively .
	manualset3
216786	9	420040	7	NULL	NULL	0	NULL	1.43 + / - 0.15	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of 0.1 mM arachidonic acid , the rate of the reduction of nitroblue tetrazolium ( NBT ) to nitroblue formazan ( NBF ) was stimulated from 0.65 + / - 0.10 to 1.43 + / - 0.15 and from 0.092 + / - 0.006 to 0.162 + / - 0.009 nmol/min/mg protein in intact and broken cell preparations , respectively .
	manualset3
216787	10	420040	7	NULL	NULL	0	NULL	 0.092 + / - 0.006	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of 0.1 mM arachidonic acid , the rate of the reduction of nitroblue tetrazolium ( NBT ) to nitroblue formazan ( NBF ) was stimulated from 0.65 + / - 0.10 to 1.43 + / - 0.15 and from 0.092 + / - 0.006 to 0.162 + / - 0.009 nmol/min/mg protein in intact and broken cell preparations , respectively .
	manualset3
216788	11	420040	7	NULL	NULL	0	NULL	0.162 + / - 0.009 nmol/min/mg protein 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of 0.1 mM arachidonic acid , the rate of the reduction of nitroblue tetrazolium ( NBT ) to nitroblue formazan ( NBF ) was stimulated from 0.65 + / - 0.10 to 1.43 + / - 0.15 and from 0.092 + / - 0.006 to 0.162 + / - 0.009 nmol/min/mg protein in intact and broken cell preparations , respectively .
	manualset3
216789	12	420040	7	NULL	NULL	0	NULL	broken cell preparations	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of 0.1 mM arachidonic acid , the rate of the reduction of nitroblue tetrazolium ( NBT ) to nitroblue formazan ( NBF ) was stimulated from 0.65 + / - 0.10 to 1.43 + / - 0.15 and from 0.092 + / - 0.006 to 0.162 + / - 0.009 nmol/min/mg protein in intact and broken cell preparations , respectively .
	manualset3
216790	1	420041	7	NULL	NULL	0	NULL	Adenylyl cyclase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenylyl cyclase was stimulated either directly using forskolin or via activation of 5-HT7 receptors .
	manualset3
216791	2	420041	7	NULL	NULL	0	NULL	forskolin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenylyl cyclase was stimulated either directly using forskolin or via activation of 5-HT7 receptors .
	manualset3
216792	3	420041	7	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenylyl cyclase was stimulated either directly using forskolin or via activation of 5-HT7 receptors .
	manualset3
216793	4	420041	7	NULL	NULL	0	NULL	5-HT7 receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenylyl cyclase was stimulated either directly using forskolin or via activation of 5-HT7 receptors .
	manualset3
216794	1	420042	7	NULL	NULL	0	NULL	dietary soybean oil level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Gradually increasing the dietary soybean oil level in the low protein diet further increased the tissue TBARS concentrations .
	manualset3
216795	2	420042	7	NULL	NULL	0	NULL	 low protein diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Gradually increasing the dietary soybean oil level in the low protein diet further increased the tissue TBARS concentrations .
	manualset3
216796	3	420042	7	NULL	NULL	0	NULL	 tissue TBARS concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Gradually increasing the dietary soybean oil level in the low protein diet further increased the tissue TBARS concentrations .
	manualset3
216797	1	420043	7	NULL	NULL	0	NULL	engineered monomer	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	An engineered monomer of CCL2 has anti-inflammatory properties emphasizing the importance of oligomerization for chemokine activity in vivo .
	manualset3
216798	2	420043	7	NULL	NULL	0	NULL	CCL2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	An engineered monomer of CCL2 has anti-inflammatory properties emphasizing the importance of oligomerization for chemokine activity in vivo .
	manualset3
216799	3	420043	7	NULL	NULL	0	NULL	anti-inflammatory properties	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An engineered monomer of CCL2 has anti-inflammatory properties emphasizing the importance of oligomerization for chemokine activity in vivo .
	manualset3
216801	5	420043	7	NULL	NULL	0	NULL	oligomerization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An engineered monomer of CCL2 has anti-inflammatory properties emphasizing the importance of oligomerization for chemokine activity in vivo .
	manualset3
216802	6	420043	7	NULL	NULL	0	NULL	chemokine activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An engineered monomer of CCL2 has anti-inflammatory properties emphasizing the importance of oligomerization for chemokine activity in vivo .
	manualset3
216803	1	420044	7	NULL	NULL	0	NULL	 experiment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This experiment is analogous to the bilinear rotation decoupling ( BIRD ) sequence in liquid-state NMR spectroscopy which selects for signals from 1H directly bound to 13C .
	manualset3
216804	2	420044	7	NULL	NULL	NULL	NULL	 bilinear rotation decoupling ( BIRD ) sequence	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This experiment is analogous to the bilinear rotation decoupling ( BIRD ) sequence in liquid-state NMR spectroscopy which selects for signals from 1H directly bound to 13C .
	manualset3
216805	3	420044	7	NULL	NULL	0	NULL	liquid-state NMR spectroscopy 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This experiment is analogous to the bilinear rotation decoupling ( BIRD ) sequence in liquid-state NMR spectroscopy which selects for signals from 1H directly bound to 13C .
	manualset3
216806	4	420044	7	NULL	NULL	0	NULL	signals	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	This experiment is analogous to the bilinear rotation decoupling ( BIRD ) sequence in liquid-state NMR spectroscopy which selects for signals from 1H directly bound to 13C .
	manualset3
216807	5	420044	7	NULL	NULL	0	NULL	1H	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	This experiment is analogous to the bilinear rotation decoupling ( BIRD ) sequence in liquid-state NMR spectroscopy which selects for signals from 1H directly bound to 13C .
	manualset3
216808	6	420044	7	NULL	NULL	0	NULL	13C	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	This experiment is analogous to the bilinear rotation decoupling ( BIRD ) sequence in liquid-state NMR spectroscopy which selects for signals from 1H directly bound to 13C .
	manualset3
216809	1	420045	7	NULL	NULL	0	NULL	Inflammatory bowel disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammatory bowel disease : does disease location at presentation predict disease course ?
	manualset3
216810	2	420045	7	NULL	NULL	0	NULL	disease location	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammatory bowel disease : does disease location at presentation predict disease course ?
	manualset3
216811	3	420045	7	NULL	NULL	0	NULL	presentation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammatory bowel disease : does disease location at presentation predict disease course ?
	manualset3
216812	4	420045	7	NULL	NULL	0	NULL	disease course	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Inflammatory bowel disease : does disease location at presentation predict disease course ?
	manualset3
216813	1	420046	7	NULL	NULL	0	NULL	 effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of nitroprusside on the secretion of pancreatic juice were investigated in preparations of isolated and blood-perfused canine pancreas .
	manualset3
216814	2	420046	7	NULL	NULL	0	NULL	nitroprusside	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of nitroprusside on the secretion of pancreatic juice were investigated in preparations of isolated and blood-perfused canine pancreas .
	manualset3
216815	3	420046	7	NULL	NULL	0	NULL	secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of nitroprusside on the secretion of pancreatic juice were investigated in preparations of isolated and blood-perfused canine pancreas .
	manualset3
216816	4	420046	7	NULL	NULL	0	NULL	pancreatic juice	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of nitroprusside on the secretion of pancreatic juice were investigated in preparations of isolated and blood-perfused canine pancreas .
	manualset3
216817	5	420046	7	NULL	NULL	0	NULL	preparations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of nitroprusside on the secretion of pancreatic juice were investigated in preparations of isolated and blood-perfused canine pancreas .
	manualset3
216818	6	420046	7	NULL	NULL	0	NULL	isolated canine pancreas 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of nitroprusside on the secretion of pancreatic juice were investigated in preparations of isolated and blood-perfused canine pancreas .
	manualset3
216819	7	420046	7	NULL	NULL	0	NULL	blood-perfused canine pancreas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of nitroprusside on the secretion of pancreatic juice were investigated in preparations of isolated and blood-perfused canine pancreas .
	manualset3
216820	1	420047	7	NULL	NULL	0	NULL	Drug-eluting stents	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug-eluting stents versus bare-metal stents for off-label indications : a propensity score-matched outcome study .
	manualset3
216821	2	420047	7	NULL	NULL	0	NULL	 bare-metal stents	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug-eluting stents versus bare-metal stents for off-label indications : a propensity score-matched outcome study .
	manualset3
216822	3	420047	7	NULL	NULL	0	NULL	off-label indications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug-eluting stents versus bare-metal stents for off-label indications : a propensity score-matched outcome study .
	manualset3
216823	4	420047	7	NULL	NULL	0	NULL	propensity score-matched outcome study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug-eluting stents versus bare-metal stents for off-label indications : a propensity score-matched outcome study .
	manualset3
216824	1	420048	7	NULL	NULL	0	NULL	liver transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The liver transplantation for hereditary ATTR amyloidosis has become a well-established treatment , because the main source of serum variant TTR is shut out .
	manualset3
216825	2	420048	7	NULL	NULL	0	NULL	hereditary ATTR amyloidosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The liver transplantation for hereditary ATTR amyloidosis has become a well-established treatment , because the main source of serum variant TTR is shut out .
	manualset3
216826	3	420048	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The liver transplantation for hereditary ATTR amyloidosis has become a well-established treatment , because the main source of serum variant TTR is shut out .
	manualset3
216827	4	420048	7	NULL	NULL	0	NULL	main source	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The liver transplantation for hereditary ATTR amyloidosis has become a well-established treatment , because the main source of serum variant TTR is shut out .
	manualset3
216828	5	420048	7	NULL	NULL	0	NULL	serum variant TTR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The liver transplantation for hereditary ATTR amyloidosis has become a well-established treatment , because the main source of serum variant TTR is shut out .
	manualset3
216829	1	420049	7	NULL	NULL	0	NULL	number of years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the number of years of life gained is high for every case of cervical cancer prevented , the disadvantages of lowering the screening age would be very large and even become disproportionate compared to the potential advantages .
	manualset3
216830	2	420049	7	NULL	NULL	0	NULL	life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the number of years of life gained is high for every case of cervical cancer prevented , the disadvantages of lowering the screening age would be very large and even become disproportionate compared to the potential advantages .
	manualset3
216831	3	420049	7	NULL	NULL	0	NULL	case	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the number of years of life gained is high for every case of cervical cancer prevented , the disadvantages of lowering the screening age would be very large and even become disproportionate compared to the potential advantages .
	manualset3
216832	4	420049	7	NULL	NULL	0	NULL	cervical cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the number of years of life gained is high for every case of cervical cancer prevented , the disadvantages of lowering the screening age would be very large and even become disproportionate compared to the potential advantages .
	manualset3
216833	5	420049	7	NULL	NULL	0	NULL	disadvantages	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the number of years of life gained is high for every case of cervical cancer prevented , the disadvantages of lowering the screening age would be very large and even become disproportionate compared to the potential advantages .
	manualset3
216834	6	420049	7	NULL	NULL	0	NULL	screening age	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the number of years of life gained is high for every case of cervical cancer prevented , the disadvantages of lowering the screening age would be very large and even become disproportionate compared to the potential advantages .
	manualset3
216835	7	420049	7	NULL	NULL	0	NULL	potential advantages	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the number of years of life gained is high for every case of cervical cancer prevented , the disadvantages of lowering the screening age would be very large and even become disproportionate compared to the potential advantages .
	manualset3
216836	1	420050	7	NULL	NULL	0	NULL	 decolorization kinetics	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The decolorization kinetics of OG by Fenton oxidation process followed the second-order reaction kinetics , and the apparent activation energy E , was detected to be 34.84 kJ mol ( -1 ) .
	manualset3
216837	2	420050	7	NULL	NULL	0	NULL	OG 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The decolorization kinetics of OG by Fenton oxidation process followed the second-order reaction kinetics , and the apparent activation energy E , was detected to be 34.84 kJ mol ( -1 ) .
	manualset3
216838	3	420050	7	NULL	NULL	0	NULL	Fenton oxidation process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The decolorization kinetics of OG by Fenton oxidation process followed the second-order reaction kinetics , and the apparent activation energy E , was detected to be 34.84 kJ mol ( -1 ) .
	manualset3
216839	4	420050	7	NULL	NULL	0	NULL	second-order reaction kinetics	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The decolorization kinetics of OG by Fenton oxidation process followed the second-order reaction kinetics , and the apparent activation energy E , was detected to be 34.84 kJ mol ( -1 ) .
	manualset3
216840	5	420050	7	NULL	NULL	NULL	NULL	activation energy E	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The decolorization kinetics of OG by Fenton oxidation process followed the second-order reaction kinetics , and the apparent activation energy E , was detected to be 34.84 kJ mol ( -1 ) .
	manualset3
216841	6	420050	7	NULL	NULL	0	NULL	34.84 kJ mol ( -1 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The decolorization kinetics of OG by Fenton oxidation process followed the second-order reaction kinetics , and the apparent activation energy E , was detected to be 34.84 kJ mol ( -1 ) .
	manualset3
216842	1	420051	7	NULL	NULL	0	NULL	glutathione	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	However , glutathione is not always a basic redox component in biological fluids , organelles , cells or tissues .
	manualset3
216843	2	420051	7	NULL	NULL	0	NULL	basic redox component 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	However , glutathione is not always a basic redox component in biological fluids , organelles , cells or tissues .
	manualset3
216844	3	420051	7	NULL	NULL	0	NULL	biological fluids	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , glutathione is not always a basic redox component in biological fluids , organelles , cells or tissues .
	manualset3
216845	4	420051	7	NULL	NULL	0	NULL	organelles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	However , glutathione is not always a basic redox component in biological fluids , organelles , cells or tissues .
	manualset3
216846	5	420051	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , glutathione is not always a basic redox component in biological fluids , organelles , cells or tissues .
	manualset3
216847	6	420051	7	NULL	NULL	0	NULL	tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	However , glutathione is not always a basic redox component in biological fluids , organelles , cells or tissues .
	manualset3
216848	1	420052	7	NULL	NULL	0	NULL	Arterioles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterioles ( 200-300 um ) were stimulated electrically to create an endothelial lesion ; ADP was then perfused for 2 min to induce the formation of a platelet-rich thrombus which lysed spontaneously in 140 + / - 24 s. Two successive ADP superfusions produced comparable thrombi which lysed in comparable times .
	manualset3
216849	2	420052	7	NULL	NULL	0	NULL	200-300 um	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterioles ( 200-300 um ) were stimulated electrically to create an endothelial lesion ; ADP was then perfused for 2 min to induce the formation of a platelet-rich thrombus which lysed spontaneously in 140 + / - 24 s. Two successive ADP superfusions produced comparable thrombi which lysed in comparable times .
	manualset3
216850	3	420052	7	NULL	NULL	0	NULL	endothelial lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterioles ( 200-300 um ) were stimulated electrically to create an endothelial lesion ; ADP was then perfused for 2 min to induce the formation of a platelet-rich thrombus which lysed spontaneously in 140 + / - 24 s. Two successive ADP superfusions produced comparable thrombi which lysed in comparable times .
	manualset3
216851	4	420052	7	NULL	NULL	0	NULL	ADP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterioles ( 200-300 um ) were stimulated electrically to create an endothelial lesion ; ADP was then perfused for 2 min to induce the formation of a platelet-rich thrombus which lysed spontaneously in 140 + / - 24 s. Two successive ADP superfusions produced comparable thrombi which lysed in comparable times .
	manualset3
216852	5	420052	7	NULL	NULL	0	NULL	2 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterioles ( 200-300 um ) were stimulated electrically to create an endothelial lesion ; ADP was then perfused for 2 min to induce the formation of a platelet-rich thrombus which lysed spontaneously in 140 + / - 24 s. Two successive ADP superfusions produced comparable thrombi which lysed in comparable times .
	manualset3
216853	6	420052	7	NULL	NULL	0	NULL	formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterioles ( 200-300 um ) were stimulated electrically to create an endothelial lesion ; ADP was then perfused for 2 min to induce the formation of a platelet-rich thrombus which lysed spontaneously in 140 + / - 24 s. Two successive ADP superfusions produced comparable thrombi which lysed in comparable times .
	manualset3
216854	7	420052	7	NULL	NULL	0	NULL	 platelet-rich thrombus	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterioles ( 200-300 um ) were stimulated electrically to create an endothelial lesion ; ADP was then perfused for 2 min to induce the formation of a platelet-rich thrombus which lysed spontaneously in 140 + / - 24 s. Two successive ADP superfusions produced comparable thrombi which lysed in comparable times .
	manualset3
216855	8	420052	7	NULL	NULL	0	NULL	140 + / - 24 s	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterioles ( 200-300 um ) were stimulated electrically to create an endothelial lesion ; ADP was then perfused for 2 min to induce the formation of a platelet-rich thrombus which lysed spontaneously in 140 + / - 24 s. Two successive ADP superfusions produced comparable thrombi which lysed in comparable times .
	manualset3
216856	9	420052	7	NULL	NULL	0	NULL	Two successive ADP superfusions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterioles ( 200-300 um ) were stimulated electrically to create an endothelial lesion ; ADP was then perfused for 2 min to induce the formation of a platelet-rich thrombus which lysed spontaneously in 140 + / - 24 s. Two successive ADP superfusions produced comparable thrombi which lysed in comparable times .
	manualset3
216857	10	420052	7	NULL	NULL	0	NULL	comparable thrombi	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterioles ( 200-300 um ) were stimulated electrically to create an endothelial lesion ; ADP was then perfused for 2 min to induce the formation of a platelet-rich thrombus which lysed spontaneously in 140 + / - 24 s. Two successive ADP superfusions produced comparable thrombi which lysed in comparable times .
	manualset3
216858	11	420052	7	NULL	NULL	0	NULL	comparable times	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterioles ( 200-300 um ) were stimulated electrically to create an endothelial lesion ; ADP was then perfused for 2 min to induce the formation of a platelet-rich thrombus which lysed spontaneously in 140 + / - 24 s. Two successive ADP superfusions produced comparable thrombi which lysed in comparable times .
	manualset3
216859	1	420053	7	NULL	NULL	0	NULL	One fragment	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	One fragment commenced with Ile at position 7 and the other with Ser at position 20 , with a cleavage point subsequent to a lysyl residue in both .
	manualset3
216860	2	420053	7	NULL	NULL	0	NULL	Ile	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	One fragment commenced with Ile at position 7 and the other with Ser at position 20 , with a cleavage point subsequent to a lysyl residue in both .
	manualset3
216861	3	420053	7	NULL	NULL	0	NULL	position 7 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	One fragment commenced with Ile at position 7 and the other with Ser at position 20 , with a cleavage point subsequent to a lysyl residue in both .
	manualset3
216862	4	420053	7	NULL	NULL	0	NULL	Ser	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	One fragment commenced with Ile at position 7 and the other with Ser at position 20 , with a cleavage point subsequent to a lysyl residue in both .
	manualset3
216863	5	420053	7	NULL	NULL	0	NULL	position 20	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	One fragment commenced with Ile at position 7 and the other with Ser at position 20 , with a cleavage point subsequent to a lysyl residue in both .
	manualset3
216864	6	420053	7	NULL	NULL	0	NULL	cleavage point 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One fragment commenced with Ile at position 7 and the other with Ser at position 20 , with a cleavage point subsequent to a lysyl residue in both .
	manualset3
216865	7	420053	7	NULL	NULL	0	NULL	lysyl residue	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	One fragment commenced with Ile at position 7 and the other with Ser at position 20 , with a cleavage point subsequent to a lysyl residue in both .
	manualset3
216866	1	420054	7	NULL	NULL	0	NULL	Comparison 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the deduced amino acid sequences of the NS and VP2 genes reveals that the virulent strains possess a 12-kDa coding NS gene and have residues Thr , Ala , Thr/Ala , and Tyr/His at positions 217 , 221 , 247 , and 500 of the VP2 gene , respectively-the motifs identified in this study to be involved in the virulence of IPNV .
	manualset3
216867	2	420054	7	NULL	NULL	0	NULL	 amino acid sequences	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the deduced amino acid sequences of the NS and VP2 genes reveals that the virulent strains possess a 12-kDa coding NS gene and have residues Thr , Ala , Thr/Ala , and Tyr/His at positions 217 , 221 , 247 , and 500 of the VP2 gene , respectively-the motifs identified in this study to be involved in the virulence of IPNV .
	manualset3
216868	3	420054	7	NULL	NULL	0	NULL	NS gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the deduced amino acid sequences of the NS and VP2 genes reveals that the virulent strains possess a 12-kDa coding NS gene and have residues Thr , Ala , Thr/Ala , and Tyr/His at positions 217 , 221 , 247 , and 500 of the VP2 gene , respectively-the motifs identified in this study to be involved in the virulence of IPNV .
	manualset3
216869	4	420054	7	NULL	NULL	0	NULL	VP2 genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the deduced amino acid sequences of the NS and VP2 genes reveals that the virulent strains possess a 12-kDa coding NS gene and have residues Thr , Ala , Thr/Ala , and Tyr/His at positions 217 , 221 , 247 , and 500 of the VP2 gene , respectively-the motifs identified in this study to be involved in the virulence of IPNV .
	manualset3
216870	5	420054	7	NULL	NULL	0	NULL	virulent strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the deduced amino acid sequences of the NS and VP2 genes reveals that the virulent strains possess a 12-kDa coding NS gene and have residues Thr , Ala , Thr/Ala , and Tyr/His at positions 217 , 221 , 247 , and 500 of the VP2 gene , respectively-the motifs identified in this study to be involved in the virulence of IPNV .
	manualset3
216871	6	420054	7	NULL	NULL	0	NULL	12-kDa 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the deduced amino acid sequences of the NS and VP2 genes reveals that the virulent strains possess a 12-kDa coding NS gene and have residues Thr , Ala , Thr/Ala , and Tyr/His at positions 217 , 221 , 247 , and 500 of the VP2 gene , respectively-the motifs identified in this study to be involved in the virulence of IPNV .
	manualset3
216872	7	420054	7	NULL	NULL	0	NULL	NS gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the deduced amino acid sequences of the NS and VP2 genes reveals that the virulent strains possess a 12-kDa coding NS gene and have residues Thr , Ala , Thr/Ala , and Tyr/His at positions 217 , 221 , 247 , and 500 of the VP2 gene , respectively-the motifs identified in this study to be involved in the virulence of IPNV .
	manualset3
216873	8	420054	7	NULL	NULL	0	NULL	residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the deduced amino acid sequences of the NS and VP2 genes reveals that the virulent strains possess a 12-kDa coding NS gene and have residues Thr , Ala , Thr/Ala , and Tyr/His at positions 217 , 221 , 247 , and 500 of the VP2 gene , respectively-the motifs identified in this study to be involved in the virulence of IPNV .
	manualset3
216874	9	420054	7	NULL	NULL	0	NULL	Thr	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the deduced amino acid sequences of the NS and VP2 genes reveals that the virulent strains possess a 12-kDa coding NS gene and have residues Thr , Ala , Thr/Ala , and Tyr/His at positions 217 , 221 , 247 , and 500 of the VP2 gene , respectively-the motifs identified in this study to be involved in the virulence of IPNV .
	manualset3
216875	10	420054	7	NULL	NULL	0	NULL	Ala	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the deduced amino acid sequences of the NS and VP2 genes reveals that the virulent strains possess a 12-kDa coding NS gene and have residues Thr , Ala , Thr/Ala , and Tyr/His at positions 217 , 221 , 247 , and 500 of the VP2 gene , respectively-the motifs identified in this study to be involved in the virulence of IPNV .
	manualset3
216876	11	420054	7	NULL	NULL	0	NULL	Thr/Ala	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the deduced amino acid sequences of the NS and VP2 genes reveals that the virulent strains possess a 12-kDa coding NS gene and have residues Thr , Ala , Thr/Ala , and Tyr/His at positions 217 , 221 , 247 , and 500 of the VP2 gene , respectively-the motifs identified in this study to be involved in the virulence of IPNV .
	manualset3
216877	12	420054	7	NULL	NULL	0	NULL	Tyr/His	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the deduced amino acid sequences of the NS and VP2 genes reveals that the virulent strains possess a 12-kDa coding NS gene and have residues Thr , Ala , Thr/Ala , and Tyr/His at positions 217 , 221 , 247 , and 500 of the VP2 gene , respectively-the motifs identified in this study to be involved in the virulence of IPNV .
	manualset3
216878	13	420054	7	NULL	NULL	0	NULL	positions	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the deduced amino acid sequences of the NS and VP2 genes reveals that the virulent strains possess a 12-kDa coding NS gene and have residues Thr , Ala , Thr/Ala , and Tyr/His at positions 217 , 221 , 247 , and 500 of the VP2 gene , respectively-the motifs identified in this study to be involved in the virulence of IPNV .
	manualset3
216879	14	420054	7	NULL	NULL	0	NULL	217	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the deduced amino acid sequences of the NS and VP2 genes reveals that the virulent strains possess a 12-kDa coding NS gene and have residues Thr , Ala , Thr/Ala , and Tyr/His at positions 217 , 221 , 247 , and 500 of the VP2 gene , respectively-the motifs identified in this study to be involved in the virulence of IPNV .
	manualset3
216880	15	420054	7	NULL	NULL	0	NULL	221	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the deduced amino acid sequences of the NS and VP2 genes reveals that the virulent strains possess a 12-kDa coding NS gene and have residues Thr , Ala , Thr/Ala , and Tyr/His at positions 217 , 221 , 247 , and 500 of the VP2 gene , respectively-the motifs identified in this study to be involved in the virulence of IPNV .
	manualset3
216881	16	420054	7	NULL	NULL	NULL	NULL	247	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Comparison of the deduced amino acid sequences of the NS and VP2 genes reveals that the virulent strains possess a 12-kDa coding NS gene and have residues Thr , Ala , Thr/Ala , and Tyr/His at positions 217 , 221 , 247 , and 500 of the VP2 gene , respectively-the motifs identified in this study to be involved in the virulence of IPNV .
	manualset3
216882	17	420054	7	NULL	NULL	0	NULL	500	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the deduced amino acid sequences of the NS and VP2 genes reveals that the virulent strains possess a 12-kDa coding NS gene and have residues Thr , Ala , Thr/Ala , and Tyr/His at positions 217 , 221 , 247 , and 500 of the VP2 gene , respectively-the motifs identified in this study to be involved in the virulence of IPNV .
	manualset3
216883	18	420054	7	NULL	NULL	0	NULL	VP2 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the deduced amino acid sequences of the NS and VP2 genes reveals that the virulent strains possess a 12-kDa coding NS gene and have residues Thr , Ala , Thr/Ala , and Tyr/His at positions 217 , 221 , 247 , and 500 of the VP2 gene , respectively-the motifs identified in this study to be involved in the virulence of IPNV .
	manualset3
216884	19	420054	7	NULL	NULL	0	NULL	 motifs	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the deduced amino acid sequences of the NS and VP2 genes reveals that the virulent strains possess a 12-kDa coding NS gene and have residues Thr , Ala , Thr/Ala , and Tyr/His at positions 217 , 221 , 247 , and 500 of the VP2 gene , respectively-the motifs identified in this study to be involved in the virulence of IPNV .
	manualset3
216885	20	420054	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the deduced amino acid sequences of the NS and VP2 genes reveals that the virulent strains possess a 12-kDa coding NS gene and have residues Thr , Ala , Thr/Ala , and Tyr/His at positions 217 , 221 , 247 , and 500 of the VP2 gene , respectively-the motifs identified in this study to be involved in the virulence of IPNV .
	manualset3
216886	21	420054	7	NULL	NULL	0	NULL	virulence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the deduced amino acid sequences of the NS and VP2 genes reveals that the virulent strains possess a 12-kDa coding NS gene and have residues Thr , Ala , Thr/Ala , and Tyr/His at positions 217 , 221 , 247 , and 500 of the VP2 gene , respectively-the motifs identified in this study to be involved in the virulence of IPNV .
	manualset3
216887	22	420054	7	NULL	NULL	0	NULL	IPNV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the deduced amino acid sequences of the NS and VP2 genes reveals that the virulent strains possess a 12-kDa coding NS gene and have residues Thr , Ala , Thr/Ala , and Tyr/His at positions 217 , 221 , 247 , and 500 of the VP2 gene , respectively-the motifs identified in this study to be involved in the virulence of IPNV .
	manualset3
216888	1	420055	7	NULL	NULL	0	NULL	high proportion 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A high proportion of the inhibitory activity shown by urine toward precipitation of ammonium acid urate is ultrafilterable and most of this can be accounted for by the common , low molecular weight components of urine .
	manualset3
216889	2	420055	7	NULL	NULL	0	NULL	inhibitory activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A high proportion of the inhibitory activity shown by urine toward precipitation of ammonium acid urate is ultrafilterable and most of this can be accounted for by the common , low molecular weight components of urine .
	manualset3
216890	3	420055	7	NULL	NULL	0	NULL	 urine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A high proportion of the inhibitory activity shown by urine toward precipitation of ammonium acid urate is ultrafilterable and most of this can be accounted for by the common , low molecular weight components of urine .
	manualset3
216891	4	420055	7	NULL	NULL	0	NULL	precipitation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A high proportion of the inhibitory activity shown by urine toward precipitation of ammonium acid urate is ultrafilterable and most of this can be accounted for by the common , low molecular weight components of urine .
	manualset3
216892	5	420055	7	NULL	NULL	0	NULL	ammonium acid urate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A high proportion of the inhibitory activity shown by urine toward precipitation of ammonium acid urate is ultrafilterable and most of this can be accounted for by the common , low molecular weight components of urine .
	manualset3
216893	6	420055	7	NULL	NULL	0	NULL	low molecular weight components	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A high proportion of the inhibitory activity shown by urine toward precipitation of ammonium acid urate is ultrafilterable and most of this can be accounted for by the common , low molecular weight components of urine .
	manualset3
216894	7	420055	7	NULL	NULL	0	NULL	urine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A high proportion of the inhibitory activity shown by urine toward precipitation of ammonium acid urate is ultrafilterable and most of this can be accounted for by the common , low molecular weight components of urine .
	manualset3
216896	1	420056	7	NULL	NULL	0	NULL	Investigation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation into the impact of obesity on immune function and long-term adverse outcomes is needed .
	manualset3
216897	2	420056	7	NULL	NULL	0	NULL	 impact	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation into the impact of obesity on immune function and long-term adverse outcomes is needed .
	manualset3
216898	3	420056	7	NULL	NULL	0	NULL	obesity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation into the impact of obesity on immune function and long-term adverse outcomes is needed .
	manualset3
216899	4	420056	7	NULL	NULL	0	NULL	immune function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation into the impact of obesity on immune function and long-term adverse outcomes is needed .
	manualset3
216900	5	420056	7	NULL	NULL	0	NULL	long-term adverse outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation into the impact of obesity on immune function and long-term adverse outcomes is needed .
	manualset3
216901	1	420057	7	NULL	NULL	0	NULL	progeny	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the progeny had simple restriction enzyme patterns unlike the viremic parents or congenitally infected progeny .
	manualset3
216902	2	420057	7	NULL	NULL	0	NULL	simple restriction enzyme patterns	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the progeny had simple restriction enzyme patterns unlike the viremic parents or congenitally infected progeny .
	manualset3
216903	3	420057	7	NULL	NULL	0	NULL	viremic parents	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the progeny had simple restriction enzyme patterns unlike the viremic parents or congenitally infected progeny .
	manualset3
216904	4	420057	7	NULL	NULL	0	NULL	congenitally infected progeny	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the progeny had simple restriction enzyme patterns unlike the viremic parents or congenitally infected progeny .
	manualset3
216905	1	420058	7	NULL	NULL	NULL	NULL	radial artery pressures	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although the other radial artery pressures and the surgeon 's estimate of systolic aortic pressure were statistically similar to the aortic root pressures , the range of differences was clinically significant .
	manualset3
216906	2	420058	7	NULL	NULL	0	NULL	surgeon 's estimate 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the other radial artery pressures and the surgeon 's estimate of systolic aortic pressure were statistically similar to the aortic root pressures , the range of differences was clinically significant .
	manualset3
216907	3	420058	7	NULL	NULL	0	NULL	systolic aortic pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the other radial artery pressures and the surgeon 's estimate of systolic aortic pressure were statistically similar to the aortic root pressures , the range of differences was clinically significant .
	manualset3
216908	4	420058	7	NULL	NULL	0	NULL	aortic root pressures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the other radial artery pressures and the surgeon 's estimate of systolic aortic pressure were statistically similar to the aortic root pressures , the range of differences was clinically significant .
	manualset3
216909	5	420058	7	NULL	NULL	0	NULL	range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the other radial artery pressures and the surgeon 's estimate of systolic aortic pressure were statistically similar to the aortic root pressures , the range of differences was clinically significant .
	manualset3
216910	6	420058	7	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the other radial artery pressures and the surgeon 's estimate of systolic aortic pressure were statistically similar to the aortic root pressures , the range of differences was clinically significant .
	manualset3
216911	1	420059	7	NULL	NULL	NULL	NULL	Seven nanosized materials	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Seven nanosized materials were tested , and chemiluminescence was detected from six of them during the catalytic oxidation of organic vapors in air .
	manualset3
216912	2	420059	7	NULL	NULL	0	NULL	chemiluminescence	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven nanosized materials were tested , and chemiluminescence was detected from six of them during the catalytic oxidation of organic vapors in air .
	manualset3
216913	3	420059	7	NULL	NULL	0	NULL	 six	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven nanosized materials were tested , and chemiluminescence was detected from six of them during the catalytic oxidation of organic vapors in air .
	manualset3
216914	4	420059	7	NULL	NULL	0	NULL	catalytic oxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven nanosized materials were tested , and chemiluminescence was detected from six of them during the catalytic oxidation of organic vapors in air .
	manualset3
216915	5	420059	7	NULL	NULL	0	NULL	 organic vapors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven nanosized materials were tested , and chemiluminescence was detected from six of them during the catalytic oxidation of organic vapors in air .
	manualset3
216916	6	420059	7	NULL	NULL	0	NULL	 air	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven nanosized materials were tested , and chemiluminescence was detected from six of them during the catalytic oxidation of organic vapors in air .
	manualset3
216917	1	420060	7	NULL	NULL	0	NULL	 impact	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , the impact of alpha E deficiency upon intestinal IEL numbers was greater at 3-4 wk of life than in younger animals , and affected the TCR alpha beta + CD8 + T cells more than the gamma delta T cells or the TCR alpha beta + CD4 + CD8 - population .
	manualset3
216918	2	420060	7	NULL	NULL	0	NULL	alpha E deficiency	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , the impact of alpha E deficiency upon intestinal IEL numbers was greater at 3-4 wk of life than in younger animals , and affected the TCR alpha beta + CD8 + T cells more than the gamma delta T cells or the TCR alpha beta + CD4 + CD8 - population .
	manualset3
216919	3	420060	7	NULL	NULL	0	NULL	intestinal IEL numbers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , the impact of alpha E deficiency upon intestinal IEL numbers was greater at 3-4 wk of life than in younger animals , and affected the TCR alpha beta + CD8 + T cells more than the gamma delta T cells or the TCR alpha beta + CD4 + CD8 - population .
	manualset3
216920	4	420060	7	NULL	NULL	0	NULL	 3-4 wk 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , the impact of alpha E deficiency upon intestinal IEL numbers was greater at 3-4 wk of life than in younger animals , and affected the TCR alpha beta + CD8 + T cells more than the gamma delta T cells or the TCR alpha beta + CD4 + CD8 - population .
	manualset3
216921	5	420060	7	NULL	NULL	0	NULL	 life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , the impact of alpha E deficiency upon intestinal IEL numbers was greater at 3-4 wk of life than in younger animals , and affected the TCR alpha beta + CD8 + T cells more than the gamma delta T cells or the TCR alpha beta + CD4 + CD8 - population .
	manualset3
216922	6	420060	7	NULL	NULL	0	NULL	younger animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , the impact of alpha E deficiency upon intestinal IEL numbers was greater at 3-4 wk of life than in younger animals , and affected the TCR alpha beta + CD8 + T cells more than the gamma delta T cells or the TCR alpha beta + CD4 + CD8 - population .
	manualset3
216923	7	420060	7	NULL	NULL	0	NULL	TCR alpha beta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , the impact of alpha E deficiency upon intestinal IEL numbers was greater at 3-4 wk of life than in younger animals , and affected the TCR alpha beta + CD8 + T cells more than the gamma delta T cells or the TCR alpha beta + CD4 + CD8 - population .
	manualset3
216924	8	420060	7	NULL	NULL	0	NULL	CD8	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , the impact of alpha E deficiency upon intestinal IEL numbers was greater at 3-4 wk of life than in younger animals , and affected the TCR alpha beta + CD8 + T cells more than the gamma delta T cells or the TCR alpha beta + CD4 + CD8 - population .
	manualset3
216925	9	420060	7	NULL	NULL	0	NULL	T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , the impact of alpha E deficiency upon intestinal IEL numbers was greater at 3-4 wk of life than in younger animals , and affected the TCR alpha beta + CD8 + T cells more than the gamma delta T cells or the TCR alpha beta + CD4 + CD8 - population .
	manualset3
216926	10	420060	7	NULL	NULL	0	NULL	gamma delta T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , the impact of alpha E deficiency upon intestinal IEL numbers was greater at 3-4 wk of life than in younger animals , and affected the TCR alpha beta + CD8 + T cells more than the gamma delta T cells or the TCR alpha beta + CD4 + CD8 - population .
	manualset3
216927	11	420060	7	NULL	NULL	0	NULL	TCR alpha beta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , the impact of alpha E deficiency upon intestinal IEL numbers was greater at 3-4 wk of life than in younger animals , and affected the TCR alpha beta + CD8 + T cells more than the gamma delta T cells or the TCR alpha beta + CD4 + CD8 - population .
	manualset3
216928	12	420060	7	NULL	NULL	0	NULL	CD4	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , the impact of alpha E deficiency upon intestinal IEL numbers was greater at 3-4 wk of life than in younger animals , and affected the TCR alpha beta + CD8 + T cells more than the gamma delta T cells or the TCR alpha beta + CD4 + CD8 - population .
	manualset3
216929	13	420060	7	NULL	NULL	0	NULL	CD8 - population	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , the impact of alpha E deficiency upon intestinal IEL numbers was greater at 3-4 wk of life than in younger animals , and affected the TCR alpha beta + CD8 + T cells more than the gamma delta T cells or the TCR alpha beta + CD4 + CD8 - population .
	manualset3
216930	1	420061	7	NULL	NULL	0	NULL	Indirect laryngoscopy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Indirect laryngoscopy was used to direct the needle , in an attempt to cover a broad area of motor end plates .
	manualset3
216931	2	420061	7	NULL	NULL	0	NULL	 needle	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Indirect laryngoscopy was used to direct the needle , in an attempt to cover a broad area of motor end plates .
	manualset3
216932	3	420061	7	NULL	NULL	0	NULL	broad area	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Indirect laryngoscopy was used to direct the needle , in an attempt to cover a broad area of motor end plates .
	manualset3
216933	4	420061	7	NULL	NULL	0	NULL	motor end plates	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Indirect laryngoscopy was used to direct the needle , in an attempt to cover a broad area of motor end plates .
	manualset3
216934	1	420062	7	NULL	NULL	0	NULL	Medical students	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical students and comprehensive patient care : attitudes , perceived competence and demonstrated ability .
	manualset3
216935	2	420062	7	NULL	NULL	0	NULL	comprehensive patient care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical students and comprehensive patient care : attitudes , perceived competence and demonstrated ability .
	manualset3
216936	3	420062	7	NULL	NULL	0	NULL	attitudes	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical students and comprehensive patient care : attitudes , perceived competence and demonstrated ability .
	manualset3
216937	4	420062	7	NULL	NULL	0	NULL	perceived competence	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical students and comprehensive patient care : attitudes , perceived competence and demonstrated ability .
	manualset3
216938	5	420062	7	NULL	NULL	0	NULL	demonstrated ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Medical students and comprehensive patient care : attitudes , perceived competence and demonstrated ability .
	manualset3
216939	1	420063	7	NULL	NULL	0	NULL	Protein recognition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein recognition by an ensemble of fluorescent DNA G-quadruplexes .
	manualset3
216940	2	420063	7	NULL	NULL	0	NULL	ensemble	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein recognition by an ensemble of fluorescent DNA G-quadruplexes .
	manualset3
216941	3	420063	7	NULL	NULL	0	NULL	fluorescent DNA G-quadruplexes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein recognition by an ensemble of fluorescent DNA G-quadruplexes .
	manualset3
216942	1	420064	7	NULL	NULL	0	NULL	histamine secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Some characteristics of histamine secretion from rat peritoneal mast cells stimulated with nerve growth factor .
	manualset3
216943	2	420064	7	NULL	NULL	0	NULL	rat peritoneal mast cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Some characteristics of histamine secretion from rat peritoneal mast cells stimulated with nerve growth factor .
	manualset3
216944	3	420064	7	NULL	NULL	0	NULL	nerve growth factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Some characteristics of histamine secretion from rat peritoneal mast cells stimulated with nerve growth factor .
	manualset3
216945	1	420065	7	NULL	NULL	0	NULL	JH1 peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	We have synthesized the JH1 peptide and coupled it to keyhole limpet hemocyanin for use as an immunogen .
	manualset3
216946	2	420065	7	NULL	NULL	0	NULL	limpet hemocyanin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We have synthesized the JH1 peptide and coupled it to keyhole limpet hemocyanin for use as an immunogen .
	manualset3
216947	3	420065	7	NULL	NULL	0	NULL	immunogen 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We have synthesized the JH1 peptide and coupled it to keyhole limpet hemocyanin for use as an immunogen .
	manualset3
216948	1	420066	7	NULL	NULL	0	NULL	observations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations strongly support the formation of an unique molecular complex of C ( 2n ) H ( 2 ) I ( 6 ) ( n = 5-7 ) upon photoabsorption by an I ( 2 ) molecule within a cluster of polyyne and iodine molecules , C ( 2n ) H ( 2 ) ( I ( 2 ) ) ( m ) ( m 3 ) .
	manualset3
216949	2	420066	7	NULL	NULL	0	NULL	formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations strongly support the formation of an unique molecular complex of C ( 2n ) H ( 2 ) I ( 6 ) ( n = 5-7 ) upon photoabsorption by an I ( 2 ) molecule within a cluster of polyyne and iodine molecules , C ( 2n ) H ( 2 ) ( I ( 2 ) ) ( m ) ( m 3 ) .
	manualset3
216950	3	420066	7	NULL	NULL	0	NULL	unique molecular complex	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations strongly support the formation of an unique molecular complex of C ( 2n ) H ( 2 ) I ( 6 ) ( n = 5-7 ) upon photoabsorption by an I ( 2 ) molecule within a cluster of polyyne and iodine molecules , C ( 2n ) H ( 2 ) ( I ( 2 ) ) ( m ) ( m 3 ) .
	manualset3
216951	4	420066	7	NULL	NULL	0	NULL	C ( 2n ) H ( 2 ) I ( 6 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations strongly support the formation of an unique molecular complex of C ( 2n ) H ( 2 ) I ( 6 ) ( n = 5-7 ) upon photoabsorption by an I ( 2 ) molecule within a cluster of polyyne and iodine molecules , C ( 2n ) H ( 2 ) ( I ( 2 ) ) ( m ) ( m 3 ) .
	manualset3
216952	5	420066	7	NULL	NULL	0	NULL	n = 5-7 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations strongly support the formation of an unique molecular complex of C ( 2n ) H ( 2 ) I ( 6 ) ( n = 5-7 ) upon photoabsorption by an I ( 2 ) molecule within a cluster of polyyne and iodine molecules , C ( 2n ) H ( 2 ) ( I ( 2 ) ) ( m ) ( m 3 ) .
	manualset3
216953	6	420066	7	NULL	NULL	0	NULL	photoabsorption	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations strongly support the formation of an unique molecular complex of C ( 2n ) H ( 2 ) I ( 6 ) ( n = 5-7 ) upon photoabsorption by an I ( 2 ) molecule within a cluster of polyyne and iodine molecules , C ( 2n ) H ( 2 ) ( I ( 2 ) ) ( m ) ( m 3 ) .
	manualset3
216954	7	420066	7	NULL	NULL	0	NULL	I ( 2 ) molecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations strongly support the formation of an unique molecular complex of C ( 2n ) H ( 2 ) I ( 6 ) ( n = 5-7 ) upon photoabsorption by an I ( 2 ) molecule within a cluster of polyyne and iodine molecules , C ( 2n ) H ( 2 ) ( I ( 2 ) ) ( m ) ( m 3 ) .
	manualset3
216955	8	420066	7	NULL	NULL	0	NULL	cluster	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations strongly support the formation of an unique molecular complex of C ( 2n ) H ( 2 ) I ( 6 ) ( n = 5-7 ) upon photoabsorption by an I ( 2 ) molecule within a cluster of polyyne and iodine molecules , C ( 2n ) H ( 2 ) ( I ( 2 ) ) ( m ) ( m 3 ) .
	manualset3
216956	9	420066	7	NULL	NULL	0	NULL	polyyne molecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations strongly support the formation of an unique molecular complex of C ( 2n ) H ( 2 ) I ( 6 ) ( n = 5-7 ) upon photoabsorption by an I ( 2 ) molecule within a cluster of polyyne and iodine molecules , C ( 2n ) H ( 2 ) ( I ( 2 ) ) ( m ) ( m 3 ) .
	manualset3
216957	10	420066	7	NULL	NULL	0	NULL	iodine molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations strongly support the formation of an unique molecular complex of C ( 2n ) H ( 2 ) I ( 6 ) ( n = 5-7 ) upon photoabsorption by an I ( 2 ) molecule within a cluster of polyyne and iodine molecules , C ( 2n ) H ( 2 ) ( I ( 2 ) ) ( m ) ( m 3 ) .
	manualset3
216958	11	420066	7	NULL	NULL	0	NULL	C ( 2n ) H ( 2 ) ( I ( 2 ) ) ( m ) ( m 3 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations strongly support the formation of an unique molecular complex of C ( 2n ) H ( 2 ) I ( 6 ) ( n = 5-7 ) upon photoabsorption by an I ( 2 ) molecule within a cluster of polyyne and iodine molecules , C ( 2n ) H ( 2 ) ( I ( 2 ) ) ( m ) ( m 3 ) .
	manualset3
216959	1	420067	7	NULL	NULL	0	NULL	Ca2 + permeability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the overall Ca2 + permeability did not vary during development , the prolonged receptor opening in the early postnatal period causes an enhanced Na + / Ca2 + influx into the immature astrocytes .
	manualset3
216960	2	420067	7	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the overall Ca2 + permeability did not vary during development , the prolonged receptor opening in the early postnatal period causes an enhanced Na + / Ca2 + influx into the immature astrocytes .
	manualset3
216961	3	420067	7	NULL	NULL	0	NULL	prolonged receptor opening	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the overall Ca2 + permeability did not vary during development , the prolonged receptor opening in the early postnatal period causes an enhanced Na + / Ca2 + influx into the immature astrocytes .
	manualset3
216962	4	420067	7	NULL	NULL	0	NULL	early postnatal period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the overall Ca2 + permeability did not vary during development , the prolonged receptor opening in the early postnatal period causes an enhanced Na + / Ca2 + influx into the immature astrocytes .
	manualset3
216963	5	420067	7	NULL	NULL	0	NULL	enhanced Na + / Ca2 + influx	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the overall Ca2 + permeability did not vary during development , the prolonged receptor opening in the early postnatal period causes an enhanced Na + / Ca2 + influx into the immature astrocytes .
	manualset3
216964	6	420067	7	NULL	NULL	0	NULL	immature astrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the overall Ca2 + permeability did not vary during development , the prolonged receptor opening in the early postnatal period causes an enhanced Na + / Ca2 + influx into the immature astrocytes .
	manualset3
216965	1	420068	7	NULL	NULL	0	NULL	Chronic pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic pain also seems related to this problem .
	manualset3
216966	2	420068	7	NULL	NULL	0	NULL	problem	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic pain also seems related to this problem .
	manualset3
216967	1	420069	7	NULL	NULL	0	NULL	LCP	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After LCP , clinical improvement was noted in 5 of 6 patients .
	manualset3
216968	2	420069	7	NULL	NULL	0	NULL	clinical improvement 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After LCP , clinical improvement was noted in 5 of 6 patients .
	manualset3
216969	3	420069	7	NULL	NULL	0	NULL	5 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	After LCP , clinical improvement was noted in 5 of 6 patients .
	manualset3
216970	4	420069	7	NULL	NULL	0	NULL	6 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	After LCP , clinical improvement was noted in 5 of 6 patients .
	manualset3
216971	1	420070	7	NULL	NULL	0	NULL	concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	At this concentration of CIPC , microtubules were distributed normally in filamentous cells .
	manualset3
216972	2	420070	7	NULL	NULL	0	NULL	CIPC	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	At this concentration of CIPC , microtubules were distributed normally in filamentous cells .
	manualset3
216973	3	420070	7	NULL	NULL	0	NULL	microtubules	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	At this concentration of CIPC , microtubules were distributed normally in filamentous cells .
	manualset3
216974	4	420070	7	NULL	NULL	0	NULL	filamentous cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	At this concentration of CIPC , microtubules were distributed normally in filamentous cells .
	manualset3
216975	1	420071	7	NULL	NULL	0	NULL	Infant death rates	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infant death rates were higher for males than for females during the early neonatal period but this difference disappeared by the end of the 1st year of life .
	manualset3
216976	2	420071	7	NULL	NULL	0	NULL	males	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Infant death rates were higher for males than for females during the early neonatal period but this difference disappeared by the end of the 1st year of life .
	manualset3
216977	3	420071	7	NULL	NULL	0	NULL	females	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Infant death rates were higher for males than for females during the early neonatal period but this difference disappeared by the end of the 1st year of life .
	manualset3
216978	4	420071	7	NULL	NULL	0	NULL	early neonatal period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Infant death rates were higher for males than for females during the early neonatal period but this difference disappeared by the end of the 1st year of life .
	manualset3
216979	5	420071	7	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Infant death rates were higher for males than for females during the early neonatal period but this difference disappeared by the end of the 1st year of life .
	manualset3
216980	6	420071	7	NULL	NULL	0	NULL	end of the 1st year 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Infant death rates were higher for males than for females during the early neonatal period but this difference disappeared by the end of the 1st year of life .
	manualset3
216981	7	420071	7	NULL	NULL	0	NULL	 life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Infant death rates were higher for males than for females during the early neonatal period but this difference disappeared by the end of the 1st year of life .
	manualset3
216982	1	420072	7	NULL	NULL	0	NULL	whole-brain blood oxygenation level-dependent ( BOLD ) functional magnetic resonance imaging data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	We obtained whole-brain blood oxygenation level-dependent ( BOLD ) functional magnetic resonance imaging data from 35 smokers during the presentation of pleasant ( erotica and romance ) , unpleasant ( mutilations and sad ) , neutral , and cigarette-related pictures .
	manualset3
216983	2	420072	7	NULL	NULL	0	NULL	35 smokers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We obtained whole-brain blood oxygenation level-dependent ( BOLD ) functional magnetic resonance imaging data from 35 smokers during the presentation of pleasant ( erotica and romance ) , unpleasant ( mutilations and sad ) , neutral , and cigarette-related pictures .
	manualset3
216984	3	420072	7	NULL	NULL	0	NULL	presentation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We obtained whole-brain blood oxygenation level-dependent ( BOLD ) functional magnetic resonance imaging data from 35 smokers during the presentation of pleasant ( erotica and romance ) , unpleasant ( mutilations and sad ) , neutral , and cigarette-related pictures .
	manualset3
216985	4	420072	7	NULL	NULL	0	NULL	pleasant pictures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We obtained whole-brain blood oxygenation level-dependent ( BOLD ) functional magnetic resonance imaging data from 35 smokers during the presentation of pleasant ( erotica and romance ) , unpleasant ( mutilations and sad ) , neutral , and cigarette-related pictures .
	manualset3
216986	5	420072	7	NULL	NULL	NULL	NULL	erotica	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We obtained whole-brain blood oxygenation level-dependent ( BOLD ) functional magnetic resonance imaging data from 35 smokers during the presentation of pleasant ( erotica and romance ) , unpleasant ( mutilations and sad ) , neutral , and cigarette-related pictures .
	manualset3
216987	6	420072	7	NULL	NULL	0	NULL	romance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We obtained whole-brain blood oxygenation level-dependent ( BOLD ) functional magnetic resonance imaging data from 35 smokers during the presentation of pleasant ( erotica and romance ) , unpleasant ( mutilations and sad ) , neutral , and cigarette-related pictures .
	manualset3
216988	7	420072	7	NULL	NULL	NULL	NULL	unpleasant pictures	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We obtained whole-brain blood oxygenation level-dependent ( BOLD ) functional magnetic resonance imaging data from 35 smokers during the presentation of pleasant ( erotica and romance ) , unpleasant ( mutilations and sad ) , neutral , and cigarette-related pictures .
	manualset3
216989	8	420072	7	NULL	NULL	0	NULL	 mutilations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We obtained whole-brain blood oxygenation level-dependent ( BOLD ) functional magnetic resonance imaging data from 35 smokers during the presentation of pleasant ( erotica and romance ) , unpleasant ( mutilations and sad ) , neutral , and cigarette-related pictures .
	manualset3
216990	9	420072	7	NULL	NULL	0	NULL	sad	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We obtained whole-brain blood oxygenation level-dependent ( BOLD ) functional magnetic resonance imaging data from 35 smokers during the presentation of pleasant ( erotica and romance ) , unpleasant ( mutilations and sad ) , neutral , and cigarette-related pictures .
	manualset3
216991	10	420072	7	NULL	NULL	0	NULL	neutral pictures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We obtained whole-brain blood oxygenation level-dependent ( BOLD ) functional magnetic resonance imaging data from 35 smokers during the presentation of pleasant ( erotica and romance ) , unpleasant ( mutilations and sad ) , neutral , and cigarette-related pictures .
	manualset3
216992	11	420072	7	NULL	NULL	0	NULL	cigarette-related pictures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We obtained whole-brain blood oxygenation level-dependent ( BOLD ) functional magnetic resonance imaging data from 35 smokers during the presentation of pleasant ( erotica and romance ) , unpleasant ( mutilations and sad ) , neutral , and cigarette-related pictures .
	manualset3
216993	1	420073	7	NULL	NULL	0	NULL	investigations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our investigations concerning the importance of cell surface macromolecules during embryonic development led us to the discovery in 1961 that heterologous anti-rat kidney serum produced teratogenesis , growth retardation and embryonic death when injected into the pregnant rat during early organogenesis .
	manualset3
216994	2	420073	7	NULL	NULL	0	NULL	cell surface macromolecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Our investigations concerning the importance of cell surface macromolecules during embryonic development led us to the discovery in 1961 that heterologous anti-rat kidney serum produced teratogenesis , growth retardation and embryonic death when injected into the pregnant rat during early organogenesis .
	manualset3
216995	3	420073	7	NULL	NULL	0	NULL	embryonic development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our investigations concerning the importance of cell surface macromolecules during embryonic development led us to the discovery in 1961 that heterologous anti-rat kidney serum produced teratogenesis , growth retardation and embryonic death when injected into the pregnant rat during early organogenesis .
	manualset3
216996	4	420073	7	NULL	NULL	0	NULL	discovery	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our investigations concerning the importance of cell surface macromolecules during embryonic development led us to the discovery in 1961 that heterologous anti-rat kidney serum produced teratogenesis , growth retardation and embryonic death when injected into the pregnant rat during early organogenesis .
	manualset3
216997	5	420073	7	NULL	NULL	0	NULL	1961	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Our investigations concerning the importance of cell surface macromolecules during embryonic development led us to the discovery in 1961 that heterologous anti-rat kidney serum produced teratogenesis , growth retardation and embryonic death when injected into the pregnant rat during early organogenesis .
	manualset3
216998	6	420073	7	NULL	NULL	0	NULL	heterologous anti-rat kidney serum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our investigations concerning the importance of cell surface macromolecules during embryonic development led us to the discovery in 1961 that heterologous anti-rat kidney serum produced teratogenesis , growth retardation and embryonic death when injected into the pregnant rat during early organogenesis .
	manualset3
216999	7	420073	7	NULL	NULL	0	NULL	teratogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our investigations concerning the importance of cell surface macromolecules during embryonic development led us to the discovery in 1961 that heterologous anti-rat kidney serum produced teratogenesis , growth retardation and embryonic death when injected into the pregnant rat during early organogenesis .
	manualset3
217000	8	420073	7	NULL	NULL	0	NULL	 growth retardation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our investigations concerning the importance of cell surface macromolecules during embryonic development led us to the discovery in 1961 that heterologous anti-rat kidney serum produced teratogenesis , growth retardation and embryonic death when injected into the pregnant rat during early organogenesis .
	manualset3
217001	9	420073	7	NULL	NULL	0	NULL	 embryonic death 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our investigations concerning the importance of cell surface macromolecules during embryonic development led us to the discovery in 1961 that heterologous anti-rat kidney serum produced teratogenesis , growth retardation and embryonic death when injected into the pregnant rat during early organogenesis .
	manualset3
217002	10	420073	7	NULL	NULL	0	NULL	pregnant rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our investigations concerning the importance of cell surface macromolecules during embryonic development led us to the discovery in 1961 that heterologous anti-rat kidney serum produced teratogenesis , growth retardation and embryonic death when injected into the pregnant rat during early organogenesis .
	manualset3
217003	11	420073	7	NULL	NULL	0	NULL	early organogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our investigations concerning the importance of cell surface macromolecules during embryonic development led us to the discovery in 1961 that heterologous anti-rat kidney serum produced teratogenesis , growth retardation and embryonic death when injected into the pregnant rat during early organogenesis .
	manualset3
217004	1	420074	7	NULL	NULL	0	NULL	changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	But the changes of the cranium were mild , only the dipole was slightly dilated .
	manualset3
217005	2	420074	7	NULL	NULL	0	NULL	cranium 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	But the changes of the cranium were mild , only the dipole was slightly dilated .
	manualset3
217006	3	420074	7	NULL	NULL	NULL	NULL	dipole	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	But the changes of the cranium were mild , only the dipole was slightly dilated .
	manualset3
217007	1	420075	7	NULL	NULL	0	NULL	mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A mechanism is proposed which involves rate-determining addition of the carbene center of A to the remote alkynyl carbon of a second alkynylcarbene complex to generate vinyl carbene intermediate C , and rearrangement of C to the enediyne complex by a ( 1 , 1.5 ) Re shift .
	manualset3
217008	2	420075	7	NULL	NULL	0	NULL	rate-determining addition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A mechanism is proposed which involves rate-determining addition of the carbene center of A to the remote alkynyl carbon of a second alkynylcarbene complex to generate vinyl carbene intermediate C , and rearrangement of C to the enediyne complex by a ( 1 , 1.5 ) Re shift .
	manualset3
217009	3	420075	7	NULL	NULL	0	NULL	carbene center	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A mechanism is proposed which involves rate-determining addition of the carbene center of A to the remote alkynyl carbon of a second alkynylcarbene complex to generate vinyl carbene intermediate C , and rearrangement of C to the enediyne complex by a ( 1 , 1.5 ) Re shift .
	manualset3
217010	4	420075	7	NULL	NULL	0	NULL	A	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A mechanism is proposed which involves rate-determining addition of the carbene center of A to the remote alkynyl carbon of a second alkynylcarbene complex to generate vinyl carbene intermediate C , and rearrangement of C to the enediyne complex by a ( 1 , 1.5 ) Re shift .
	manualset3
217011	5	420075	7	NULL	NULL	0	NULL	alkynyl carbon	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	A mechanism is proposed which involves rate-determining addition of the carbene center of A to the remote alkynyl carbon of a second alkynylcarbene complex to generate vinyl carbene intermediate C , and rearrangement of C to the enediyne complex by a ( 1 , 1.5 ) Re shift .
	manualset3
217012	6	420075	7	NULL	NULL	0	NULL	second alkynylcarbene complex	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A mechanism is proposed which involves rate-determining addition of the carbene center of A to the remote alkynyl carbon of a second alkynylcarbene complex to generate vinyl carbene intermediate C , and rearrangement of C to the enediyne complex by a ( 1 , 1.5 ) Re shift .
	manualset3
217013	7	420075	7	NULL	NULL	0	NULL	 vinyl carbene intermediate C	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A mechanism is proposed which involves rate-determining addition of the carbene center of A to the remote alkynyl carbon of a second alkynylcarbene complex to generate vinyl carbene intermediate C , and rearrangement of C to the enediyne complex by a ( 1 , 1.5 ) Re shift .
	manualset3
217014	8	420075	7	NULL	NULL	0	NULL	 rearrangement of C	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A mechanism is proposed which involves rate-determining addition of the carbene center of A to the remote alkynyl carbon of a second alkynylcarbene complex to generate vinyl carbene intermediate C , and rearrangement of C to the enediyne complex by a ( 1 , 1.5 ) Re shift .
	manualset3
217015	9	420075	7	NULL	NULL	0	NULL	enediyne complex	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A mechanism is proposed which involves rate-determining addition of the carbene center of A to the remote alkynyl carbon of a second alkynylcarbene complex to generate vinyl carbene intermediate C , and rearrangement of C to the enediyne complex by a ( 1 , 1.5 ) Re shift .
	manualset3
217016	10	420075	7	NULL	NULL	0	NULL	( 1 , 1.5 ) Re shift	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A mechanism is proposed which involves rate-determining addition of the carbene center of A to the remote alkynyl carbon of a second alkynylcarbene complex to generate vinyl carbene intermediate C , and rearrangement of C to the enediyne complex by a ( 1 , 1.5 ) Re shift .
	manualset3
217017	1	420076	7	NULL	NULL	0	NULL	purpose	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our purpose was to characterize the spectrum of hepatobiliary abnormalities on sonography in children with vertically transmitted HIV infection .
	manualset3
217018	2	420076	7	NULL	NULL	0	NULL	spectrum	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our purpose was to characterize the spectrum of hepatobiliary abnormalities on sonography in children with vertically transmitted HIV infection .
	manualset3
217019	3	420076	7	NULL	NULL	0	NULL	hepatobiliary abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our purpose was to characterize the spectrum of hepatobiliary abnormalities on sonography in children with vertically transmitted HIV infection .
	manualset3
217020	4	420076	7	NULL	NULL	0	NULL	sonography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Our purpose was to characterize the spectrum of hepatobiliary abnormalities on sonography in children with vertically transmitted HIV infection .
	manualset3
217021	5	420076	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our purpose was to characterize the spectrum of hepatobiliary abnormalities on sonography in children with vertically transmitted HIV infection .
	manualset3
217022	6	420076	7	NULL	NULL	0	NULL	vertically transmitted HIV infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our purpose was to characterize the spectrum of hepatobiliary abnormalities on sonography in children with vertically transmitted HIV infection .
	manualset3
217023	1	420077	7	NULL	NULL	0	NULL	Matching chemistry	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Matching chemistry and shape in molecular docking .
	manualset3
217024	2	420077	7	NULL	NULL	0	NULL	shape	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Matching chemistry and shape in molecular docking .
	manualset3
217025	3	420077	7	NULL	NULL	0	NULL	molecular docking	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Matching chemistry and shape in molecular docking .
	manualset3
217026	1	420078	7	NULL	NULL	0	NULL	cytosolic fraction	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A cytosolic fraction prepared from a mouse fibroblast cell line reduced secondary products of lipid peroxidation , including alkenals , alkanals , alk-2-enals , and alka-2 , 4 - dienals , using NADH or NADPH .
	manualset3
217027	2	420078	7	NULL	NULL	0	NULL	mouse fibroblast cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A cytosolic fraction prepared from a mouse fibroblast cell line reduced secondary products of lipid peroxidation , including alkenals , alkanals , alk-2-enals , and alka-2 , 4 - dienals , using NADH or NADPH .
	manualset3
217028	3	420078	7	NULL	NULL	0	NULL	secondary products	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A cytosolic fraction prepared from a mouse fibroblast cell line reduced secondary products of lipid peroxidation , including alkenals , alkanals , alk-2-enals , and alka-2 , 4 - dienals , using NADH or NADPH .
	manualset3
217029	4	420078	7	NULL	NULL	0	NULL	lipid peroxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A cytosolic fraction prepared from a mouse fibroblast cell line reduced secondary products of lipid peroxidation , including alkenals , alkanals , alk-2-enals , and alka-2 , 4 - dienals , using NADH or NADPH .
	manualset3
217030	5	420078	7	NULL	NULL	0	NULL	alkenals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A cytosolic fraction prepared from a mouse fibroblast cell line reduced secondary products of lipid peroxidation , including alkenals , alkanals , alk-2-enals , and alka-2 , 4 - dienals , using NADH or NADPH .
	manualset3
217031	6	420078	7	NULL	NULL	0	NULL	alkanals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A cytosolic fraction prepared from a mouse fibroblast cell line reduced secondary products of lipid peroxidation , including alkenals , alkanals , alk-2-enals , and alka-2 , 4 - dienals , using NADH or NADPH .
	manualset3
217032	7	420078	7	NULL	NULL	0	NULL	alk-2-enals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A cytosolic fraction prepared from a mouse fibroblast cell line reduced secondary products of lipid peroxidation , including alkenals , alkanals , alk-2-enals , and alka-2 , 4 - dienals , using NADH or NADPH .
	manualset3
217033	8	420078	7	NULL	NULL	0	NULL	alka-2 , 4 - dienals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A cytosolic fraction prepared from a mouse fibroblast cell line reduced secondary products of lipid peroxidation , including alkenals , alkanals , alk-2-enals , and alka-2 , 4 - dienals , using NADH or NADPH .
	manualset3
217034	9	420078	7	NULL	NULL	0	NULL	NADH	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A cytosolic fraction prepared from a mouse fibroblast cell line reduced secondary products of lipid peroxidation , including alkenals , alkanals , alk-2-enals , and alka-2 , 4 - dienals , using NADH or NADPH .
	manualset3
217035	10	420078	7	NULL	NULL	0	NULL	NADPH	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A cytosolic fraction prepared from a mouse fibroblast cell line reduced secondary products of lipid peroxidation , including alkenals , alkanals , alk-2-enals , and alka-2 , 4 - dienals , using NADH or NADPH .
	manualset3
217036	1	420079	7	NULL	NULL	0	NULL	family study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A family study of coronary risk factors in Geelong .
	manualset3
217037	2	420079	7	NULL	NULL	0	NULL	coronary risk factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A family study of coronary risk factors in Geelong .
	manualset3
217038	3	420079	7	NULL	NULL	0	NULL	Geelong	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A family study of coronary risk factors in Geelong .
	manualset3
217039	1	420080	7	NULL	NULL	0	NULL	yeast actin cytoskeleton	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We characterized the yeast actin cytoskeleton at the ultrastructural level using immunoelectron microscopy .
	manualset3
217040	2	420080	7	NULL	NULL	0	NULL	ultrastructural level	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We characterized the yeast actin cytoskeleton at the ultrastructural level using immunoelectron microscopy .
	manualset3
217041	3	420080	7	NULL	NULL	0	NULL	immunoelectron microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We characterized the yeast actin cytoskeleton at the ultrastructural level using immunoelectron microscopy .
	manualset3
217122	1	420081	7	NULL	NULL	NULL	NULL	Sensitive and specific thin-layer ( TLC ) methods	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Sensitive and specific thin-layer ( TLC ) and high-performance liquid chromatographic ( HPLC ) methods were developed for the determination of the diuretic agent 2-chloro-5 - ( 4-hydroxy-3-methyl-2 - ( methylimino ) -4 - thiazolidinyl ) benzenesulphonamide hydrochloride ( HOE 740 ) .
	manualset3
217123	2	420081	7	NULL	NULL	0	NULL	high-performance liquid chromatographic ( HPLC ) methods 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitive and specific thin-layer ( TLC ) and high-performance liquid chromatographic ( HPLC ) methods were developed for the determination of the diuretic agent 2-chloro-5 - ( 4-hydroxy-3-methyl-2 - ( methylimino ) -4 - thiazolidinyl ) benzenesulphonamide hydrochloride ( HOE 740 ) .
	manualset3
217124	3	420081	7	NULL	NULL	0	NULL	determination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitive and specific thin-layer ( TLC ) and high-performance liquid chromatographic ( HPLC ) methods were developed for the determination of the diuretic agent 2-chloro-5 - ( 4-hydroxy-3-methyl-2 - ( methylimino ) -4 - thiazolidinyl ) benzenesulphonamide hydrochloride ( HOE 740 ) .
	manualset3
217125	4	420081	7	NULL	NULL	0	NULL	diuretic agent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitive and specific thin-layer ( TLC ) and high-performance liquid chromatographic ( HPLC ) methods were developed for the determination of the diuretic agent 2-chloro-5 - ( 4-hydroxy-3-methyl-2 - ( methylimino ) -4 - thiazolidinyl ) benzenesulphonamide hydrochloride ( HOE 740 ) .
	manualset3
217126	5	420081	7	NULL	NULL	0	NULL	2-chloro-5 - ( 4-hydroxy-3-methyl-2 - ( methylimino ) -4 - thiazolidinyl ) benzenesulphonamide hydrochloride ( HOE 740 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Sensitive and specific thin-layer ( TLC ) and high-performance liquid chromatographic ( HPLC ) methods were developed for the determination of the diuretic agent 2-chloro-5 - ( 4-hydroxy-3-methyl-2 - ( methylimino ) -4 - thiazolidinyl ) benzenesulphonamide hydrochloride ( HOE 740 ) .
	manualset3
217127	1	420082	7	NULL	NULL	0	NULL	major bleed	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No major bleed occurred ( a bleed which caused discontinuation of therapy , hospitalization or death ) .
	manualset3
217128	2	420082	7	NULL	NULL	0	NULL	bleed	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No major bleed occurred ( a bleed which caused discontinuation of therapy , hospitalization or death ) .
	manualset3
217129	3	420082	7	NULL	NULL	0	NULL	discontinuation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No major bleed occurred ( a bleed which caused discontinuation of therapy , hospitalization or death ) .
	manualset3
217130	4	420082	7	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	No major bleed occurred ( a bleed which caused discontinuation of therapy , hospitalization or death ) .
	manualset3
217131	5	420082	7	NULL	NULL	0	NULL	hospitalization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	No major bleed occurred ( a bleed which caused discontinuation of therapy , hospitalization or death ) .
	manualset3
217132	6	420082	7	NULL	NULL	0	NULL	death 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No major bleed occurred ( a bleed which caused discontinuation of therapy , hospitalization or death ) .
	manualset3
217133	1	420083	7	NULL	NULL	0	NULL	 patterns of staining	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the patterns of staining by lead hydroxide alone and by uranyl acetate were similar in tissues fixed for longer times ( ( 1/2 ) hour to 2 hours , at 0 degrees C or 20 degrees C ) , in briefly fixed material the DNA-containing regions appeared relatively unstained by lead hydroxide alone , whilst often there was appreciable staining of RNA-containing structures .
	manualset3
217134	2	420083	7	NULL	NULL	0	NULL	lead hydroxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the patterns of staining by lead hydroxide alone and by uranyl acetate were similar in tissues fixed for longer times ( ( 1/2 ) hour to 2 hours , at 0 degrees C or 20 degrees C ) , in briefly fixed material the DNA-containing regions appeared relatively unstained by lead hydroxide alone , whilst often there was appreciable staining of RNA-containing structures .
	manualset3
217135	3	420083	7	NULL	NULL	0	NULL	uranyl acetate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the patterns of staining by lead hydroxide alone and by uranyl acetate were similar in tissues fixed for longer times ( ( 1/2 ) hour to 2 hours , at 0 degrees C or 20 degrees C ) , in briefly fixed material the DNA-containing regions appeared relatively unstained by lead hydroxide alone , whilst often there was appreciable staining of RNA-containing structures .
	manualset3
217136	4	420083	7	NULL	NULL	0	NULL	tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the patterns of staining by lead hydroxide alone and by uranyl acetate were similar in tissues fixed for longer times ( ( 1/2 ) hour to 2 hours , at 0 degrees C or 20 degrees C ) , in briefly fixed material the DNA-containing regions appeared relatively unstained by lead hydroxide alone , whilst often there was appreciable staining of RNA-containing structures .
	manualset3
217137	5	420083	7	NULL	NULL	0	NULL	 longer times	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the patterns of staining by lead hydroxide alone and by uranyl acetate were similar in tissues fixed for longer times ( ( 1/2 ) hour to 2 hours , at 0 degrees C or 20 degrees C ) , in briefly fixed material the DNA-containing regions appeared relatively unstained by lead hydroxide alone , whilst often there was appreciable staining of RNA-containing structures .
	manualset3
217138	6	420083	7	NULL	NULL	0	NULL	( ( 1/2 ) hour	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the patterns of staining by lead hydroxide alone and by uranyl acetate were similar in tissues fixed for longer times ( ( 1/2 ) hour to 2 hours , at 0 degrees C or 20 degrees C ) , in briefly fixed material the DNA-containing regions appeared relatively unstained by lead hydroxide alone , whilst often there was appreciable staining of RNA-containing structures .
	manualset3
217139	7	420083	7	NULL	NULL	0	NULL	2 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the patterns of staining by lead hydroxide alone and by uranyl acetate were similar in tissues fixed for longer times ( ( 1/2 ) hour to 2 hours , at 0 degrees C or 20 degrees C ) , in briefly fixed material the DNA-containing regions appeared relatively unstained by lead hydroxide alone , whilst often there was appreciable staining of RNA-containing structures .
	manualset3
217140	8	420083	7	NULL	NULL	0	NULL	0 degrees C	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the patterns of staining by lead hydroxide alone and by uranyl acetate were similar in tissues fixed for longer times ( ( 1/2 ) hour to 2 hours , at 0 degrees C or 20 degrees C ) , in briefly fixed material the DNA-containing regions appeared relatively unstained by lead hydroxide alone , whilst often there was appreciable staining of RNA-containing structures .
	manualset3
217141	9	420083	7	NULL	NULL	0	NULL	20 degrees C 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the patterns of staining by lead hydroxide alone and by uranyl acetate were similar in tissues fixed for longer times ( ( 1/2 ) hour to 2 hours , at 0 degrees C or 20 degrees C ) , in briefly fixed material the DNA-containing regions appeared relatively unstained by lead hydroxide alone , whilst often there was appreciable staining of RNA-containing structures .
	manualset3
217142	10	420083	7	NULL	NULL	0	NULL	fixed material 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the patterns of staining by lead hydroxide alone and by uranyl acetate were similar in tissues fixed for longer times ( ( 1/2 ) hour to 2 hours , at 0 degrees C or 20 degrees C ) , in briefly fixed material the DNA-containing regions appeared relatively unstained by lead hydroxide alone , whilst often there was appreciable staining of RNA-containing structures .
	manualset3
217143	11	420083	7	NULL	NULL	0	NULL	DNA-containing regions	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the patterns of staining by lead hydroxide alone and by uranyl acetate were similar in tissues fixed for longer times ( ( 1/2 ) hour to 2 hours , at 0 degrees C or 20 degrees C ) , in briefly fixed material the DNA-containing regions appeared relatively unstained by lead hydroxide alone , whilst often there was appreciable staining of RNA-containing structures .
	manualset3
217144	12	420083	7	NULL	NULL	0	NULL	lead hydroxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the patterns of staining by lead hydroxide alone and by uranyl acetate were similar in tissues fixed for longer times ( ( 1/2 ) hour to 2 hours , at 0 degrees C or 20 degrees C ) , in briefly fixed material the DNA-containing regions appeared relatively unstained by lead hydroxide alone , whilst often there was appreciable staining of RNA-containing structures .
	manualset3
217145	13	420083	7	NULL	NULL	0	NULL	staining 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the patterns of staining by lead hydroxide alone and by uranyl acetate were similar in tissues fixed for longer times ( ( 1/2 ) hour to 2 hours , at 0 degrees C or 20 degrees C ) , in briefly fixed material the DNA-containing regions appeared relatively unstained by lead hydroxide alone , whilst often there was appreciable staining of RNA-containing structures .
	manualset3
217146	14	420083	7	NULL	NULL	0	NULL	RNA-containing structures	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the patterns of staining by lead hydroxide alone and by uranyl acetate were similar in tissues fixed for longer times ( ( 1/2 ) hour to 2 hours , at 0 degrees C or 20 degrees C ) , in briefly fixed material the DNA-containing regions appeared relatively unstained by lead hydroxide alone , whilst often there was appreciable staining of RNA-containing structures .
	manualset3
217147	1	420084	7	NULL	NULL	0	NULL	 GC-induced increase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The GC-induced increase in contractility was found to be consistent with an increase in F-actin content .
	manualset3
217148	2	420084	7	NULL	NULL	NULL	NULL	contractility	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The GC-induced increase in contractility was found to be consistent with an increase in F-actin content .
	manualset3
217149	3	420084	7	NULL	NULL	0	NULL	increase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The GC-induced increase in contractility was found to be consistent with an increase in F-actin content .
	manualset3
217150	4	420084	7	NULL	NULL	0	NULL	F-actin content 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The GC-induced increase in contractility was found to be consistent with an increase in F-actin content .
	manualset3
217151	1	420085	7	NULL	NULL	0	NULL	GPCRs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	GPCRs are the focus of a significant amount of current pharmaceutical research since they interact with more than 50 % of prescription drugs , whereas they still comprise the best potential targets for drug design .
	manualset3
217152	2	420085	7	NULL	NULL	0	NULL	significant amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	GPCRs are the focus of a significant amount of current pharmaceutical research since they interact with more than 50 % of prescription drugs , whereas they still comprise the best potential targets for drug design .
	manualset3
217153	3	420085	7	NULL	NULL	0	NULL	current pharmaceutical research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	GPCRs are the focus of a significant amount of current pharmaceutical research since they interact with more than 50 % of prescription drugs , whereas they still comprise the best potential targets for drug design .
	manualset3
217154	4	420085	7	NULL	NULL	0	NULL	50 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	GPCRs are the focus of a significant amount of current pharmaceutical research since they interact with more than 50 % of prescription drugs , whereas they still comprise the best potential targets for drug design .
	manualset3
217155	5	420085	7	NULL	NULL	0	NULL	prescription drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	GPCRs are the focus of a significant amount of current pharmaceutical research since they interact with more than 50 % of prescription drugs , whereas they still comprise the best potential targets for drug design .
	manualset3
217156	6	420085	7	NULL	NULL	0	NULL	best potential targets	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	GPCRs are the focus of a significant amount of current pharmaceutical research since they interact with more than 50 % of prescription drugs , whereas they still comprise the best potential targets for drug design .
	manualset3
217157	7	420085	7	NULL	NULL	0	NULL	drug design	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	GPCRs are the focus of a significant amount of current pharmaceutical research since they interact with more than 50 % of prescription drugs , whereas they still comprise the best potential targets for drug design .
	manualset3
217158	1	420086	7	NULL	NULL	0	NULL	Administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Administration of intravenous methylprednisolone ( 1g per day , 3 days ) followed by 40 mg per day of prednisolone achieved complete response , and MPO-ANCA level was decreased .
	manualset3
217159	2	420086	7	NULL	NULL	0	NULL	 methylprednisolone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Administration of intravenous methylprednisolone ( 1g per day , 3 days ) followed by 40 mg per day of prednisolone achieved complete response , and MPO-ANCA level was decreased .
	manualset3
217160	3	420086	7	NULL	NULL	0	NULL	1g per day 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Administration of intravenous methylprednisolone ( 1g per day , 3 days ) followed by 40 mg per day of prednisolone achieved complete response , and MPO-ANCA level was decreased .
	manualset3
217161	4	420086	7	NULL	NULL	0	NULL	3 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Administration of intravenous methylprednisolone ( 1g per day , 3 days ) followed by 40 mg per day of prednisolone achieved complete response , and MPO-ANCA level was decreased .
	manualset3
217162	5	420086	7	NULL	NULL	0	NULL	40 mg per day	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Administration of intravenous methylprednisolone ( 1g per day , 3 days ) followed by 40 mg per day of prednisolone achieved complete response , and MPO-ANCA level was decreased .
	manualset3
217163	6	420086	7	NULL	NULL	0	NULL	prednisolone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Administration of intravenous methylprednisolone ( 1g per day , 3 days ) followed by 40 mg per day of prednisolone achieved complete response , and MPO-ANCA level was decreased .
	manualset3
217164	7	420086	7	NULL	NULL	0	NULL	MPO-ANCA level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Administration of intravenous methylprednisolone ( 1g per day , 3 days ) followed by 40 mg per day of prednisolone achieved complete response , and MPO-ANCA level was decreased .
	manualset3
217165	8	420086	7	NULL	NULL	0	NULL	complete response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Administration of intravenous methylprednisolone ( 1g per day , 3 days ) followed by 40 mg per day of prednisolone achieved complete response , and MPO-ANCA level was decreased .
	manualset3
217166	1	420087	7	NULL	NULL	0	NULL	 first study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This is the first study to show a relationship between coffee drinking and diabetes in a Brazilian population .
	manualset3
217167	2	420087	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	This is the first study to show a relationship between coffee drinking and diabetes in a Brazilian population .
	manualset3
217168	3	420087	7	NULL	NULL	0	NULL	coffee drinking	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This is the first study to show a relationship between coffee drinking and diabetes in a Brazilian population .
	manualset3
217169	4	420087	7	NULL	NULL	0	NULL	diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This is the first study to show a relationship between coffee drinking and diabetes in a Brazilian population .
	manualset3
217170	5	420087	7	NULL	NULL	0	NULL	Brazilian population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This is the first study to show a relationship between coffee drinking and diabetes in a Brazilian population .
	manualset3
217171	1	420088	7	NULL	NULL	0	NULL	Glomerular filtration rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Glomerular filtration rate measured in this group of animals was reduced in the obstructed kidney by about 60 % compared to the contralateral one .
	manualset3
217172	2	420088	7	NULL	NULL	0	NULL	group 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Glomerular filtration rate measured in this group of animals was reduced in the obstructed kidney by about 60 % compared to the contralateral one .
	manualset3
217173	3	420088	7	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Glomerular filtration rate measured in this group of animals was reduced in the obstructed kidney by about 60 % compared to the contralateral one .
	manualset3
217174	4	420088	7	NULL	NULL	0	NULL	obstructed kidney	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Glomerular filtration rate measured in this group of animals was reduced in the obstructed kidney by about 60 % compared to the contralateral one .
	manualset3
217175	5	420088	7	NULL	NULL	0	NULL	60 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Glomerular filtration rate measured in this group of animals was reduced in the obstructed kidney by about 60 % compared to the contralateral one .
	manualset3
217176	6	420088	7	NULL	NULL	0	NULL	contralateral one	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Glomerular filtration rate measured in this group of animals was reduced in the obstructed kidney by about 60 % compared to the contralateral one .
	manualset3
217177	1	420089	7	NULL	NULL	NULL	NULL	Mesiodistal sections	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mesiodistal sections through Class II MOD restorations with the same combinations of materials after 24 hours of storage in pigment solutions and without loading revealed that a close marginal fit in the area of the cervical step can be obtained with the use of glass ionomer cement as base material .
	manualset3
217178	2	420089	7	NULL	NULL	0	NULL	Class II MOD restorations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesiodistal sections through Class II MOD restorations with the same combinations of materials after 24 hours of storage in pigment solutions and without loading revealed that a close marginal fit in the area of the cervical step can be obtained with the use of glass ionomer cement as base material .
	manualset3
217179	3	420089	7	NULL	NULL	0	NULL	same combinations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesiodistal sections through Class II MOD restorations with the same combinations of materials after 24 hours of storage in pigment solutions and without loading revealed that a close marginal fit in the area of the cervical step can be obtained with the use of glass ionomer cement as base material .
	manualset3
217180	4	420089	7	NULL	NULL	0	NULL	materials	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesiodistal sections through Class II MOD restorations with the same combinations of materials after 24 hours of storage in pigment solutions and without loading revealed that a close marginal fit in the area of the cervical step can be obtained with the use of glass ionomer cement as base material .
	manualset3
217181	5	420089	7	NULL	NULL	0	NULL	24 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesiodistal sections through Class II MOD restorations with the same combinations of materials after 24 hours of storage in pigment solutions and without loading revealed that a close marginal fit in the area of the cervical step can be obtained with the use of glass ionomer cement as base material .
	manualset3
217182	6	420089	7	NULL	NULL	0	NULL	storage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesiodistal sections through Class II MOD restorations with the same combinations of materials after 24 hours of storage in pigment solutions and without loading revealed that a close marginal fit in the area of the cervical step can be obtained with the use of glass ionomer cement as base material .
	manualset3
217183	7	420089	7	NULL	NULL	0	NULL	pigment solutions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesiodistal sections through Class II MOD restorations with the same combinations of materials after 24 hours of storage in pigment solutions and without loading revealed that a close marginal fit in the area of the cervical step can be obtained with the use of glass ionomer cement as base material .
	manualset3
217184	8	420089	7	NULL	NULL	0	NULL	loading	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesiodistal sections through Class II MOD restorations with the same combinations of materials after 24 hours of storage in pigment solutions and without loading revealed that a close marginal fit in the area of the cervical step can be obtained with the use of glass ionomer cement as base material .
	manualset3
217185	9	420089	7	NULL	NULL	0	NULL	close marginal fit	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesiodistal sections through Class II MOD restorations with the same combinations of materials after 24 hours of storage in pigment solutions and without loading revealed that a close marginal fit in the area of the cervical step can be obtained with the use of glass ionomer cement as base material .
	manualset3
217186	10	420089	7	NULL	NULL	0	NULL	area of the cervical step	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesiodistal sections through Class II MOD restorations with the same combinations of materials after 24 hours of storage in pigment solutions and without loading revealed that a close marginal fit in the area of the cervical step can be obtained with the use of glass ionomer cement as base material .
	manualset3
217187	11	420089	7	NULL	NULL	0	NULL	use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesiodistal sections through Class II MOD restorations with the same combinations of materials after 24 hours of storage in pigment solutions and without loading revealed that a close marginal fit in the area of the cervical step can be obtained with the use of glass ionomer cement as base material .
	manualset3
217188	12	420089	7	NULL	NULL	0	NULL	glass ionomer cement 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesiodistal sections through Class II MOD restorations with the same combinations of materials after 24 hours of storage in pigment solutions and without loading revealed that a close marginal fit in the area of the cervical step can be obtained with the use of glass ionomer cement as base material .
	manualset3
217189	13	420089	7	NULL	NULL	0	NULL	base material 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Mesiodistal sections through Class II MOD restorations with the same combinations of materials after 24 hours of storage in pigment solutions and without loading revealed that a close marginal fit in the area of the cervical step can be obtained with the use of glass ionomer cement as base material .
	manualset3
217190	1	420090	7	NULL	NULL	0	NULL	Pectoralis major composite flap	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pectoralis major composite flap was used in 33 patients on musculovascular pedicle and 1 patient had a latissimus dorsi composite flap free-tissue transfer .
	manualset3
217191	2	420090	7	NULL	NULL	0	NULL	 33 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Pectoralis major composite flap was used in 33 patients on musculovascular pedicle and 1 patient had a latissimus dorsi composite flap free-tissue transfer .
	manualset3
217192	3	420090	7	NULL	NULL	0	NULL	musculovascular pedicle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Pectoralis major composite flap was used in 33 patients on musculovascular pedicle and 1 patient had a latissimus dorsi composite flap free-tissue transfer .
	manualset3
217193	4	420090	7	NULL	NULL	0	NULL	1 patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Pectoralis major composite flap was used in 33 patients on musculovascular pedicle and 1 patient had a latissimus dorsi composite flap free-tissue transfer .
	manualset3
217194	5	420090	7	NULL	NULL	0	NULL	latissimus dorsi composite flap free-tissue transfer	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pectoralis major composite flap was used in 33 patients on musculovascular pedicle and 1 patient had a latissimus dorsi composite flap free-tissue transfer .
	manualset3
217195	1	420091	7	NULL	NULL	0	NULL	Involvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of human plasma angiotensin I-converting enzyme in the degradation of the hemoregulatory peptide N-acetyl-seryl-aspartyl-lysyl-proline .
	manualset3
217196	2	420091	7	NULL	NULL	0	NULL	human plasma angiotensin I-converting enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of human plasma angiotensin I-converting enzyme in the degradation of the hemoregulatory peptide N-acetyl-seryl-aspartyl-lysyl-proline .
	manualset3
217197	3	420091	7	NULL	NULL	0	NULL	degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of human plasma angiotensin I-converting enzyme in the degradation of the hemoregulatory peptide N-acetyl-seryl-aspartyl-lysyl-proline .
	manualset3
217198	4	420091	7	NULL	NULL	0	NULL	hemoregulatory peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of human plasma angiotensin I-converting enzyme in the degradation of the hemoregulatory peptide N-acetyl-seryl-aspartyl-lysyl-proline .
	manualset3
217199	5	420091	7	NULL	NULL	0	NULL	N-acetyl-seryl-aspartyl-lysyl-proline	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Involvement of human plasma angiotensin I-converting enzyme in the degradation of the hemoregulatory peptide N-acetyl-seryl-aspartyl-lysyl-proline .
	manualset3
217200	1	420092	7	NULL	NULL	NULL	NULL	periosteal MS	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although the periosteal MS/BS , MAR , and BFR/BS increased , the endosteal MS/BS , MAR , and BFR/BS decreased .
	manualset3
217201	2	420092	7	NULL	NULL	NULL	NULL	periosteal BS	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although the periosteal MS/BS , MAR , and BFR/BS increased , the endosteal MS/BS , MAR , and BFR/BS decreased .
	manualset3
217202	3	420092	7	NULL	NULL	0	NULL	MAR	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the periosteal MS/BS , MAR , and BFR/BS increased , the endosteal MS/BS , MAR , and BFR/BS decreased .
	manualset3
217203	4	420092	7	NULL	NULL	0	NULL	BFR	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the periosteal MS/BS , MAR , and BFR/BS increased , the endosteal MS/BS , MAR , and BFR/BS decreased .
	manualset3
217204	5	420092	7	NULL	NULL	0	NULL	BS	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the periosteal MS/BS , MAR , and BFR/BS increased , the endosteal MS/BS , MAR , and BFR/BS decreased .
	manualset3
217205	6	420092	7	NULL	NULL	0	NULL	endosteal MS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the periosteal MS/BS , MAR , and BFR/BS increased , the endosteal MS/BS , MAR , and BFR/BS decreased .
	manualset3
217206	7	420092	7	NULL	NULL	0	NULL	endosteal BS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the periosteal MS/BS , MAR , and BFR/BS increased , the endosteal MS/BS , MAR , and BFR/BS decreased .
	manualset3
217207	8	420092	7	NULL	NULL	0	NULL	MAR	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the periosteal MS/BS , MAR , and BFR/BS increased , the endosteal MS/BS , MAR , and BFR/BS decreased .
	manualset3
217208	9	420092	7	NULL	NULL	0	NULL	BFR/BS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the periosteal MS/BS , MAR , and BFR/BS increased , the endosteal MS/BS , MAR , and BFR/BS decreased .
	manualset3
217209	1	420093	7	NULL	NULL	0	NULL	second study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second study , a markedly better NI antibody response to the influenza A virus component was seen following immunization with split-virus vaccine , but the HAI antibody response to both split and whole vaccines was the same .
	manualset3
217210	2	420093	7	NULL	NULL	0	NULL	NI antibody response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second study , a markedly better NI antibody response to the influenza A virus component was seen following immunization with split-virus vaccine , but the HAI antibody response to both split and whole vaccines was the same .
	manualset3
217211	3	420093	7	NULL	NULL	0	NULL	influenza A virus component	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second study , a markedly better NI antibody response to the influenza A virus component was seen following immunization with split-virus vaccine , but the HAI antibody response to both split and whole vaccines was the same .
	manualset3
217212	4	420093	7	NULL	NULL	0	NULL	immunization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second study , a markedly better NI antibody response to the influenza A virus component was seen following immunization with split-virus vaccine , but the HAI antibody response to both split and whole vaccines was the same .
	manualset3
217213	5	420093	7	NULL	NULL	0	NULL	split-virus vaccine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second study , a markedly better NI antibody response to the influenza A virus component was seen following immunization with split-virus vaccine , but the HAI antibody response to both split and whole vaccines was the same .
	manualset3
217214	6	420093	7	NULL	NULL	0	NULL	HAI antibody response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second study , a markedly better NI antibody response to the influenza A virus component was seen following immunization with split-virus vaccine , but the HAI antibody response to both split and whole vaccines was the same .
	manualset3
217215	7	420093	7	NULL	NULL	0	NULL	split vaccines	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second study , a markedly better NI antibody response to the influenza A virus component was seen following immunization with split-virus vaccine , but the HAI antibody response to both split and whole vaccines was the same .
	manualset3
217216	8	420093	7	NULL	NULL	0	NULL	whole vaccines	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the second study , a markedly better NI antibody response to the influenza A virus component was seen following immunization with split-virus vaccine , but the HAI antibody response to both split and whole vaccines was the same .
	manualset3
217217	1	420094	7	NULL	NULL	0	NULL	observed isotope effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The observed isotope effects are interpreted in terms of the competitive reactions of two dihydride intermediates and dideuteride intermediates that exist in equilibrium in the catalytic cycle .
	manualset3
217218	2	420094	7	NULL	NULL	0	NULL	terms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The observed isotope effects are interpreted in terms of the competitive reactions of two dihydride intermediates and dideuteride intermediates that exist in equilibrium in the catalytic cycle .
	manualset3
217219	3	420094	7	NULL	NULL	0	NULL	competitive reactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The observed isotope effects are interpreted in terms of the competitive reactions of two dihydride intermediates and dideuteride intermediates that exist in equilibrium in the catalytic cycle .
	manualset3
217220	4	420094	7	NULL	NULL	0	NULL	two dihydride intermediates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The observed isotope effects are interpreted in terms of the competitive reactions of two dihydride intermediates and dideuteride intermediates that exist in equilibrium in the catalytic cycle .
	manualset3
217221	5	420094	7	NULL	NULL	0	NULL	dideuteride intermediates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The observed isotope effects are interpreted in terms of the competitive reactions of two dihydride intermediates and dideuteride intermediates that exist in equilibrium in the catalytic cycle .
	manualset3
217222	6	420094	7	NULL	NULL	0	NULL	equilibrium 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The observed isotope effects are interpreted in terms of the competitive reactions of two dihydride intermediates and dideuteride intermediates that exist in equilibrium in the catalytic cycle .
	manualset3
217223	7	420094	7	NULL	NULL	0	NULL	catalytic cycle	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The observed isotope effects are interpreted in terms of the competitive reactions of two dihydride intermediates and dideuteride intermediates that exist in equilibrium in the catalytic cycle .
	manualset3
217224	1	420095	7	NULL	NULL	0	NULL	Prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of disordered eating in girls : a survey of middle-class children .
	manualset3
217225	2	420095	7	NULL	NULL	0	NULL	disordered eating 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of disordered eating in girls : a survey of middle-class children .
	manualset3
217226	3	420095	7	NULL	NULL	0	NULL	girls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of disordered eating in girls : a survey of middle-class children .
	manualset3
217227	4	420095	7	NULL	NULL	0	NULL	survey	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of disordered eating in girls : a survey of middle-class children .
	manualset3
217228	5	420095	7	NULL	NULL	0	NULL	middle-class children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevalence of disordered eating in girls : a survey of middle-class children .
	manualset3
217229	1	420096	7	NULL	NULL	0	NULL	C-HO inter-action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A C-HO inter-action occurs in the crystal .
	manualset3
217230	2	420096	7	NULL	NULL	0	NULL	crystal 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A C-HO inter-action occurs in the crystal .
	manualset3
217231	1	420097	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of maximally effective concentrations of okadaic acid and/or microcystin , deactivation of the enhanced Cl - conductance upon washout of agonist was incomplete , with about half of the conductance persisting indefinitely .
	manualset3
217232	2	420097	7	NULL	NULL	0	NULL	maximally effective concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of maximally effective concentrations of okadaic acid and/or microcystin , deactivation of the enhanced Cl - conductance upon washout of agonist was incomplete , with about half of the conductance persisting indefinitely .
	manualset3
217233	3	420097	7	NULL	NULL	0	NULL	okadaic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of maximally effective concentrations of okadaic acid and/or microcystin , deactivation of the enhanced Cl - conductance upon washout of agonist was incomplete , with about half of the conductance persisting indefinitely .
	manualset3
217234	4	420097	7	NULL	NULL	0	NULL	microcystin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of maximally effective concentrations of okadaic acid and/or microcystin , deactivation of the enhanced Cl - conductance upon washout of agonist was incomplete , with about half of the conductance persisting indefinitely .
	manualset3
217235	5	420097	7	NULL	NULL	0	NULL	deactivation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of maximally effective concentrations of okadaic acid and/or microcystin , deactivation of the enhanced Cl - conductance upon washout of agonist was incomplete , with about half of the conductance persisting indefinitely .
	manualset3
217236	6	420097	7	NULL	NULL	0	NULL	enhanced Cl - conductance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of maximally effective concentrations of okadaic acid and/or microcystin , deactivation of the enhanced Cl - conductance upon washout of agonist was incomplete , with about half of the conductance persisting indefinitely .
	manualset3
217237	7	420097	7	NULL	NULL	0	NULL	washout	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of maximally effective concentrations of okadaic acid and/or microcystin , deactivation of the enhanced Cl - conductance upon washout of agonist was incomplete , with about half of the conductance persisting indefinitely .
	manualset3
217238	8	420097	7	NULL	NULL	0	NULL	agonist	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of maximally effective concentrations of okadaic acid and/or microcystin , deactivation of the enhanced Cl - conductance upon washout of agonist was incomplete , with about half of the conductance persisting indefinitely .
	manualset3
217239	9	420097	7	NULL	NULL	NULL	NULL	 half of the conductance	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the presence of maximally effective concentrations of okadaic acid and/or microcystin , deactivation of the enhanced Cl - conductance upon washout of agonist was incomplete , with about half of the conductance persisting indefinitely .
	manualset3
217240	1	420098	7	NULL	NULL	0	NULL	V. fluvialis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	V. fluvialis was recovered from the stools of 10 patients who presented clinically with gastroenteritis , from a wound in one patient , and from a caecostomy drainage specimen in one patient .
	manualset3
217241	2	420098	7	NULL	NULL	NULL	NULL	stools	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	V. fluvialis was recovered from the stools of 10 patients who presented clinically with gastroenteritis , from a wound in one patient , and from a caecostomy drainage specimen in one patient .
	manualset3
217242	3	420098	7	NULL	NULL	0	NULL	10 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	V. fluvialis was recovered from the stools of 10 patients who presented clinically with gastroenteritis , from a wound in one patient , and from a caecostomy drainage specimen in one patient .
	manualset3
217243	4	420098	7	NULL	NULL	0	NULL	gastroenteritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	V. fluvialis was recovered from the stools of 10 patients who presented clinically with gastroenteritis , from a wound in one patient , and from a caecostomy drainage specimen in one patient .
	manualset3
217244	5	420098	7	NULL	NULL	0	NULL	wound	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	V. fluvialis was recovered from the stools of 10 patients who presented clinically with gastroenteritis , from a wound in one patient , and from a caecostomy drainage specimen in one patient .
	manualset3
217245	6	420098	7	NULL	NULL	0	NULL	 one patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	V. fluvialis was recovered from the stools of 10 patients who presented clinically with gastroenteritis , from a wound in one patient , and from a caecostomy drainage specimen in one patient .
	manualset3
217246	7	420098	7	NULL	NULL	0	NULL	caecostomy drainage specimen	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	V. fluvialis was recovered from the stools of 10 patients who presented clinically with gastroenteritis , from a wound in one patient , and from a caecostomy drainage specimen in one patient .
	manualset3
217247	8	420098	7	NULL	NULL	0	NULL	one patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	V. fluvialis was recovered from the stools of 10 patients who presented clinically with gastroenteritis , from a wound in one patient , and from a caecostomy drainage specimen in one patient .
	manualset3
217248	1	420099	7	NULL	NULL	0	NULL	Lymphocyte costimulatory receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocyte costimulatory receptors in renal disease and transplantation .
	manualset3
217249	2	420099	7	NULL	NULL	0	NULL	renal disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocyte costimulatory receptors in renal disease and transplantation .
	manualset3
217250	3	420099	7	NULL	NULL	0	NULL	transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphocyte costimulatory receptors in renal disease and transplantation .
	manualset3
217251	1	420100	7	NULL	NULL	0	NULL	process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the process of physical map building has been facilitated by the flow of data released by the Human Genome Project , gathering all the information together requires significant effort .
	manualset3
217252	2	420100	7	NULL	NULL	0	NULL	physical map building	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the process of physical map building has been facilitated by the flow of data released by the Human Genome Project , gathering all the information together requires significant effort .
	manualset3
217253	3	420100	7	NULL	NULL	0	NULL	 flow of data	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the process of physical map building has been facilitated by the flow of data released by the Human Genome Project , gathering all the information together requires significant effort .
	manualset3
217254	4	420100	7	NULL	NULL	0	NULL	Human Genome Project	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the process of physical map building has been facilitated by the flow of data released by the Human Genome Project , gathering all the information together requires significant effort .
	manualset3
217255	5	420100	7	NULL	NULL	0	NULL	information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the process of physical map building has been facilitated by the flow of data released by the Human Genome Project , gathering all the information together requires significant effort .
	manualset3
217256	6	420100	7	NULL	NULL	0	NULL	 effort 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the process of physical map building has been facilitated by the flow of data released by the Human Genome Project , gathering all the information together requires significant effort .
	manualset3
217257	1	420101	7	NULL	NULL	0	NULL	Mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality developed in two patients , who were transferred after first aid in the field hospital and were in shock status on arrival to emergency department of the back-up hospital .
	manualset3
217258	2	420101	7	NULL	NULL	0	NULL	two patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality developed in two patients , who were transferred after first aid in the field hospital and were in shock status on arrival to emergency department of the back-up hospital .
	manualset3
217259	3	420101	7	NULL	NULL	0	NULL	first aid	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality developed in two patients , who were transferred after first aid in the field hospital and were in shock status on arrival to emergency department of the back-up hospital .
	manualset3
217260	4	420101	7	NULL	NULL	0	NULL	 field hospital	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality developed in two patients , who were transferred after first aid in the field hospital and were in shock status on arrival to emergency department of the back-up hospital .
	manualset3
217261	5	420101	7	NULL	NULL	0	NULL	shock status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality developed in two patients , who were transferred after first aid in the field hospital and were in shock status on arrival to emergency department of the back-up hospital .
	manualset3
217262	6	420101	7	NULL	NULL	0	NULL	arrival	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality developed in two patients , who were transferred after first aid in the field hospital and were in shock status on arrival to emergency department of the back-up hospital .
	manualset3
217263	7	420101	7	NULL	NULL	0	NULL	emergency department 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality developed in two patients , who were transferred after first aid in the field hospital and were in shock status on arrival to emergency department of the back-up hospital .
	manualset3
217264	8	420101	7	NULL	NULL	0	NULL	back-up hospital	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Mortality developed in two patients , who were transferred after first aid in the field hospital and were in shock status on arrival to emergency department of the back-up hospital .
	manualset3
217265	1	420102	7	NULL	NULL	0	NULL	detergent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the detergent did not affect chaperone-enhanced aggregation , suggesting that this aggregation does not depend on hydrophobic interactions .
	manualset3
217266	2	420102	7	NULL	NULL	NULL	NULL	chaperone-enhanced aggregation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , the detergent did not affect chaperone-enhanced aggregation , suggesting that this aggregation does not depend on hydrophobic interactions .
	manualset3
217267	3	420102	7	NULL	NULL	0	NULL	aggregation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the detergent did not affect chaperone-enhanced aggregation , suggesting that this aggregation does not depend on hydrophobic interactions .
	manualset3
217268	4	420102	7	NULL	NULL	0	NULL	hydrophobic interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the detergent did not affect chaperone-enhanced aggregation , suggesting that this aggregation does not depend on hydrophobic interactions .
	manualset3
217269	1	420103	7	NULL	NULL	0	NULL	Life-sustaining treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Life-sustaining treatment may legitimately be forgone if it is ( a ) therapeutically futile , ( b ) overly burdensome to the patient , ( c ) not reasonably available without disproportionate hardship to the patient 's carers or others , or ( d ) refused by the patient .
	manualset3
217270	2	420103	7	NULL	NULL	0	NULL	therapeutically futile	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Life-sustaining treatment may legitimately be forgone if it is ( a ) therapeutically futile , ( b ) overly burdensome to the patient , ( c ) not reasonably available without disproportionate hardship to the patient 's carers or others , or ( d ) refused by the patient .
	manualset3
217271	3	420103	7	NULL	NULL	0	NULL	overly burdensome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Life-sustaining treatment may legitimately be forgone if it is ( a ) therapeutically futile , ( b ) overly burdensome to the patient , ( c ) not reasonably available without disproportionate hardship to the patient 's carers or others , or ( d ) refused by the patient .
	manualset3
217272	4	420103	7	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Life-sustaining treatment may legitimately be forgone if it is ( a ) therapeutically futile , ( b ) overly burdensome to the patient , ( c ) not reasonably available without disproportionate hardship to the patient 's carers or others , or ( d ) refused by the patient .
	manualset3
217273	5	420103	7	NULL	NULL	0	NULL	disproportionate hardship 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Life-sustaining treatment may legitimately be forgone if it is ( a ) therapeutically futile , ( b ) overly burdensome to the patient , ( c ) not reasonably available without disproportionate hardship to the patient 's carers or others , or ( d ) refused by the patient .
	manualset3
217274	6	420103	7	NULL	NULL	0	NULL	patient 's carers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Life-sustaining treatment may legitimately be forgone if it is ( a ) therapeutically futile , ( b ) overly burdensome to the patient , ( c ) not reasonably available without disproportionate hardship to the patient 's carers or others , or ( d ) refused by the patient .
	manualset3
217275	7	420103	7	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Life-sustaining treatment may legitimately be forgone if it is ( a ) therapeutically futile , ( b ) overly burdensome to the patient , ( c ) not reasonably available without disproportionate hardship to the patient 's carers or others , or ( d ) refused by the patient .
	manualset3
217276	1	420104	7	NULL	NULL	0	NULL	discontinuous nature	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The discontinuous nature of the basement membrane in these cells may provide a clue as to the malignant nature of this tumor .
	manualset3
217277	2	420104	7	NULL	NULL	NULL	NULL	basement membrane 	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The discontinuous nature of the basement membrane in these cells may provide a clue as to the malignant nature of this tumor .
	manualset3
217278	3	420104	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The discontinuous nature of the basement membrane in these cells may provide a clue as to the malignant nature of this tumor .
	manualset3
217279	4	420104	7	NULL	NULL	0	NULL	malignant nature	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The discontinuous nature of the basement membrane in these cells may provide a clue as to the malignant nature of this tumor .
	manualset3
217280	5	420104	7	NULL	NULL	0	NULL	 tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The discontinuous nature of the basement membrane in these cells may provide a clue as to the malignant nature of this tumor .
	manualset3
217281	6	420104	7	NULL	NULL	0	NULL	 clue	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The discontinuous nature of the basement membrane in these cells may provide a clue as to the malignant nature of this tumor .
	manualset3
217282	1	420105	7	NULL	NULL	0	NULL	Evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence for non-specific brain dysfunction is often found in autism and autistic-like conditions .
	manualset3
217283	2	420105	7	NULL	NULL	0	NULL	non-specific brain dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence for non-specific brain dysfunction is often found in autism and autistic-like conditions .
	manualset3
217284	3	420105	7	NULL	NULL	0	NULL	autism	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence for non-specific brain dysfunction is often found in autism and autistic-like conditions .
	manualset3
217285	4	420105	7	NULL	NULL	0	NULL	autistic-like conditions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence for non-specific brain dysfunction is often found in autism and autistic-like conditions .
	manualset3
217286	1	420106	7	NULL	NULL	0	NULL	range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A range of noise levels from 35 to 80 dB SPL was used .
	manualset3
217287	2	420106	7	NULL	NULL	0	NULL	noise levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A range of noise levels from 35 to 80 dB SPL was used .
	manualset3
217288	3	420106	7	NULL	NULL	0	NULL	35 dB SPL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A range of noise levels from 35 to 80 dB SPL was used .
	manualset3
217289	4	420106	7	NULL	NULL	0	NULL	 80 dB SPL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A range of noise levels from 35 to 80 dB SPL was used .
	manualset3
217290	1	420107	7	NULL	NULL	0	NULL	 L isozyme contribution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The L isozyme contribution is augmented upon weaning and is sustained until the rat is adult and a L/M ratio of 9 : 1 is maintained .
	manualset3
217291	2	420107	7	NULL	NULL	0	NULL	weaning	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The L isozyme contribution is augmented upon weaning and is sustained until the rat is adult and a L/M ratio of 9 : 1 is maintained .
	manualset3
217292	3	420107	7	NULL	NULL	0	NULL	rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The L isozyme contribution is augmented upon weaning and is sustained until the rat is adult and a L/M ratio of 9 : 1 is maintained .
	manualset3
217293	4	420107	7	NULL	NULL	0	NULL	adult 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The L isozyme contribution is augmented upon weaning and is sustained until the rat is adult and a L/M ratio of 9 : 1 is maintained .
	manualset3
217294	5	420107	7	NULL	NULL	0	NULL	L/M ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The L isozyme contribution is augmented upon weaning and is sustained until the rat is adult and a L/M ratio of 9 : 1 is maintained .
	manualset3
217295	6	420107	7	NULL	NULL	0	NULL	 9 : 1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The L isozyme contribution is augmented upon weaning and is sustained until the rat is adult and a L/M ratio of 9 : 1 is maintained .
	manualset3
217296	1	420108	7	NULL	NULL	0	NULL	ability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of Vibrio vulnificus to acquire iron from the host has been shown to correlate with virulence .
	manualset3
217297	2	420108	7	NULL	NULL	0	NULL	Vibrio vulnificus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of Vibrio vulnificus to acquire iron from the host has been shown to correlate with virulence .
	manualset3
217298	3	420108	7	NULL	NULL	0	NULL	 iron	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of Vibrio vulnificus to acquire iron from the host has been shown to correlate with virulence .
	manualset3
217299	4	420108	7	NULL	NULL	0	NULL	host	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of Vibrio vulnificus to acquire iron from the host has been shown to correlate with virulence .
	manualset3
217300	5	420108	7	NULL	NULL	0	NULL	virulence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of Vibrio vulnificus to acquire iron from the host has been shown to correlate with virulence .
	manualset3
217301	1	420109	7	NULL	NULL	0	NULL	progestogen-only minipill 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the progestogen-only minipill decreases side effects such as dizziness , nausea , headaches , and breast tenderness associated with combined oral contraceptives , this advantage is outweighed by disturbances of menstrual flow .
	manualset3
217302	2	420109	7	NULL	NULL	0	NULL	 side effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the progestogen-only minipill decreases side effects such as dizziness , nausea , headaches , and breast tenderness associated with combined oral contraceptives , this advantage is outweighed by disturbances of menstrual flow .
	manualset3
217303	3	420109	7	NULL	NULL	0	NULL	dizziness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the progestogen-only minipill decreases side effects such as dizziness , nausea , headaches , and breast tenderness associated with combined oral contraceptives , this advantage is outweighed by disturbances of menstrual flow .
	manualset3
217304	4	420109	7	NULL	NULL	0	NULL	nausea	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the progestogen-only minipill decreases side effects such as dizziness , nausea , headaches , and breast tenderness associated with combined oral contraceptives , this advantage is outweighed by disturbances of menstrual flow .
	manualset3
217305	5	420109	7	NULL	NULL	0	NULL	headaches	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the progestogen-only minipill decreases side effects such as dizziness , nausea , headaches , and breast tenderness associated with combined oral contraceptives , this advantage is outweighed by disturbances of menstrual flow .
	manualset3
217306	6	420109	7	NULL	NULL	0	NULL	breast tenderness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the progestogen-only minipill decreases side effects such as dizziness , nausea , headaches , and breast tenderness associated with combined oral contraceptives , this advantage is outweighed by disturbances of menstrual flow .
	manualset3
217307	7	420109	7	NULL	NULL	0	NULL	combined oral contraceptives	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the progestogen-only minipill decreases side effects such as dizziness , nausea , headaches , and breast tenderness associated with combined oral contraceptives , this advantage is outweighed by disturbances of menstrual flow .
	manualset3
217308	8	420109	7	NULL	NULL	0	NULL	advantage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the progestogen-only minipill decreases side effects such as dizziness , nausea , headaches , and breast tenderness associated with combined oral contraceptives , this advantage is outweighed by disturbances of menstrual flow .
	manualset3
217309	9	420109	7	NULL	NULL	0	NULL	disturbances	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the progestogen-only minipill decreases side effects such as dizziness , nausea , headaches , and breast tenderness associated with combined oral contraceptives , this advantage is outweighed by disturbances of menstrual flow .
	manualset3
217310	10	420109	7	NULL	NULL	0	NULL	menstrual flow	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the progestogen-only minipill decreases side effects such as dizziness , nausea , headaches , and breast tenderness associated with combined oral contraceptives , this advantage is outweighed by disturbances of menstrual flow .
	manualset3
217311	1	420110	7	NULL	NULL	0	NULL	proposed method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed method treats training data selection as an optimization problem and involves application of a genetic algorithm ( GA ) .
	manualset3
217312	2	420110	7	NULL	NULL	0	NULL	training data selection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed method treats training data selection as an optimization problem and involves application of a genetic algorithm ( GA ) .
	manualset3
217313	3	420110	7	NULL	NULL	0	NULL	optimization problem 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed method treats training data selection as an optimization problem and involves application of a genetic algorithm ( GA ) .
	manualset3
217314	4	420110	7	NULL	NULL	0	NULL	application	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed method treats training data selection as an optimization problem and involves application of a genetic algorithm ( GA ) .
	manualset3
217315	5	420110	7	NULL	NULL	0	NULL	genetic algorithm ( GA ) 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The proposed method treats training data selection as an optimization problem and involves application of a genetic algorithm ( GA ) .
	manualset3
217316	1	420111	7	NULL	NULL	0	NULL	 isolated steroids	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolated steroids were identified by comparison with the synthetic steroids using ultraviolet and mass spectroscopy and by gas chromatography-mass spectroscopy .
	manualset3
217317	2	420111	7	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolated steroids were identified by comparison with the synthetic steroids using ultraviolet and mass spectroscopy and by gas chromatography-mass spectroscopy .
	manualset3
217318	3	420111	7	NULL	NULL	0	NULL	synthetic steroids	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolated steroids were identified by comparison with the synthetic steroids using ultraviolet and mass spectroscopy and by gas chromatography-mass spectroscopy .
	manualset3
217319	4	420111	7	NULL	NULL	0	NULL	ultraviolet spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolated steroids were identified by comparison with the synthetic steroids using ultraviolet and mass spectroscopy and by gas chromatography-mass spectroscopy .
	manualset3
217320	5	420111	7	NULL	NULL	0	NULL	mass spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolated steroids were identified by comparison with the synthetic steroids using ultraviolet and mass spectroscopy and by gas chromatography-mass spectroscopy .
	manualset3
217321	6	420111	7	NULL	NULL	0	NULL	gas chromatography-mass spectroscopy 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The isolated steroids were identified by comparison with the synthetic steroids using ultraviolet and mass spectroscopy and by gas chromatography-mass spectroscopy .
	manualset3
217322	1	420112	7	NULL	NULL	0	NULL	Role 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Role of liver pathology in the development of occupational dermatoses ( experimental studies ) ) .
	manualset3
217323	2	420112	7	NULL	NULL	0	NULL	liver pathology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Role of liver pathology in the development of occupational dermatoses ( experimental studies ) ) .
	manualset3
217324	3	420112	7	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Role of liver pathology in the development of occupational dermatoses ( experimental studies ) ) .
	manualset3
217325	4	420112	7	NULL	NULL	0	NULL	occupational dermatoses	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Role of liver pathology in the development of occupational dermatoses ( experimental studies ) ) .
	manualset3
217326	5	420112	7	NULL	NULL	0	NULL	experimental studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Role of liver pathology in the development of occupational dermatoses ( experimental studies ) ) .
	manualset3
217327	1	420113	7	NULL	NULL	0	NULL	Laser speckle velocimetry 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Laser speckle velocimetry of retinal blood flow with simultaneous measurement of retinal vessel diameter ) .
	manualset3
217328	2	420113	7	NULL	NULL	0	NULL	retinal blood flow	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Laser speckle velocimetry of retinal blood flow with simultaneous measurement of retinal vessel diameter ) .
	manualset3
217329	3	420113	7	NULL	NULL	NULL	NULL	 measurement	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Laser speckle velocimetry of retinal blood flow with simultaneous measurement of retinal vessel diameter ) .
	manualset3
217330	4	420113	7	NULL	NULL	NULL	NULL	retinal vessel diameter	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Laser speckle velocimetry of retinal blood flow with simultaneous measurement of retinal vessel diameter ) .
	manualset3
217331	1	420114	7	NULL	NULL	0	NULL	Europe	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In Europe , infections caused by the highly pathogenic avian influenza A ( H7N7 ) virus were confirmed in the human population in 2003 in the Netherlands .
	manualset3
217332	2	420114	7	NULL	NULL	0	NULL	infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In Europe , infections caused by the highly pathogenic avian influenza A ( H7N7 ) virus were confirmed in the human population in 2003 in the Netherlands .
	manualset3
217333	3	420114	7	NULL	NULL	0	NULL	highly pathogenic avian influenza A ( H7N7 ) virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In Europe , infections caused by the highly pathogenic avian influenza A ( H7N7 ) virus were confirmed in the human population in 2003 in the Netherlands .
	manualset3
217334	4	420114	7	NULL	NULL	0	NULL	human population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In Europe , infections caused by the highly pathogenic avian influenza A ( H7N7 ) virus were confirmed in the human population in 2003 in the Netherlands .
	manualset3
217335	5	420114	7	NULL	NULL	NULL	NULL	2003	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In Europe , infections caused by the highly pathogenic avian influenza A ( H7N7 ) virus were confirmed in the human population in 2003 in the Netherlands .
	manualset3
217336	6	420114	7	NULL	NULL	0	NULL	Netherlands	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In Europe , infections caused by the highly pathogenic avian influenza A ( H7N7 ) virus were confirmed in the human population in 2003 in the Netherlands .
	manualset3
217337	1	420115	7	NULL	NULL	0	NULL	gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene encoding D-ribulokinase , designated darK , was found to map within the L-fucose regulon , and the partial gene order was found to be Tn10-fucA-darK-fucI-fucK-thyA .
	manualset3
217338	2	420115	7	NULL	NULL	0	NULL	D-ribulokinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene encoding D-ribulokinase , designated darK , was found to map within the L-fucose regulon , and the partial gene order was found to be Tn10-fucA-darK-fucI-fucK-thyA .
	manualset3
217339	3	420115	7	NULL	NULL	0	NULL	darK 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene encoding D-ribulokinase , designated darK , was found to map within the L-fucose regulon , and the partial gene order was found to be Tn10-fucA-darK-fucI-fucK-thyA .
	manualset3
217340	4	420115	7	NULL	NULL	0	NULL	L-fucose regulon	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene encoding D-ribulokinase , designated darK , was found to map within the L-fucose regulon , and the partial gene order was found to be Tn10-fucA-darK-fucI-fucK-thyA .
	manualset3
217341	5	420115	7	NULL	NULL	0	NULL	partial gene order	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene encoding D-ribulokinase , designated darK , was found to map within the L-fucose regulon , and the partial gene order was found to be Tn10-fucA-darK-fucI-fucK-thyA .
	manualset3
217343	6	420115	7	NULL	NULL	0	NULL	Tn10-fucA-darK-fucI-fucK-thyA	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene encoding D-ribulokinase , designated darK , was found to map within the L-fucose regulon , and the partial gene order was found to be Tn10-fucA-darK-fucI-fucK-thyA .
	manualset3
217344	1	420116	7	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The number of episodes of jumping during the 30 min after injection of naloxone was considered as the intensity of the withdrawal syndrome .
	manualset3
217345	2	420116	7	NULL	NULL	0	NULL	episodes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The number of episodes of jumping during the 30 min after injection of naloxone was considered as the intensity of the withdrawal syndrome .
	manualset3
217346	3	420116	7	NULL	NULL	0	NULL	 jumping	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The number of episodes of jumping during the 30 min after injection of naloxone was considered as the intensity of the withdrawal syndrome .
	manualset3
217347	4	420116	7	NULL	NULL	0	NULL	30 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The number of episodes of jumping during the 30 min after injection of naloxone was considered as the intensity of the withdrawal syndrome .
	manualset3
217348	5	420116	7	NULL	NULL	0	NULL	injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The number of episodes of jumping during the 30 min after injection of naloxone was considered as the intensity of the withdrawal syndrome .
	manualset3
217349	6	420116	7	NULL	NULL	0	NULL	naloxone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The number of episodes of jumping during the 30 min after injection of naloxone was considered as the intensity of the withdrawal syndrome .
	manualset3
217350	7	420116	7	NULL	NULL	0	NULL	intensity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The number of episodes of jumping during the 30 min after injection of naloxone was considered as the intensity of the withdrawal syndrome .
	manualset3
217351	8	420116	7	NULL	NULL	0	NULL	withdrawal syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The number of episodes of jumping during the 30 min after injection of naloxone was considered as the intensity of the withdrawal syndrome .
	manualset3
217352	1	420117	7	NULL	NULL	0	NULL	Damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Damage of macular ganglion cell complex and peripapillary retinal nerve fiber layer in multiple sclerosis ) .
	manualset3
217353	2	420117	7	NULL	NULL	0	NULL	macular ganglion cell complex	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	( Damage of macular ganglion cell complex and peripapillary retinal nerve fiber layer in multiple sclerosis ) .
	manualset3
217354	3	420117	7	NULL	NULL	0	NULL	peripapillary retinal nerve fiber layer	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Damage of macular ganglion cell complex and peripapillary retinal nerve fiber layer in multiple sclerosis ) .
	manualset3
217355	4	420117	7	NULL	NULL	0	NULL	multiple sclerosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Damage of macular ganglion cell complex and peripapillary retinal nerve fiber layer in multiple sclerosis ) .
	manualset3
217356	1	420118	7	NULL	NULL	0	NULL	 receptor	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the receptor was only phosphorylated to 15 % of its maximum with 0.1 unit/ml erythropoietin , this was sufficient to induce peak hemoglobin synthesis .
	manualset3
217357	2	420118	7	NULL	NULL	0	NULL	15 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the receptor was only phosphorylated to 15 % of its maximum with 0.1 unit/ml erythropoietin , this was sufficient to induce peak hemoglobin synthesis .
	manualset3
217358	3	420118	7	NULL	NULL	0	NULL	maximum	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the receptor was only phosphorylated to 15 % of its maximum with 0.1 unit/ml erythropoietin , this was sufficient to induce peak hemoglobin synthesis .
	manualset3
217359	4	420118	7	NULL	NULL	0	NULL	 0.1 unit/ml	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the receptor was only phosphorylated to 15 % of its maximum with 0.1 unit/ml erythropoietin , this was sufficient to induce peak hemoglobin synthesis .
	manualset3
217360	5	420118	7	NULL	NULL	0	NULL	erythropoietin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the receptor was only phosphorylated to 15 % of its maximum with 0.1 unit/ml erythropoietin , this was sufficient to induce peak hemoglobin synthesis .
	manualset3
217361	6	420118	7	NULL	NULL	0	NULL	peak hemoglobin synthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the receptor was only phosphorylated to 15 % of its maximum with 0.1 unit/ml erythropoietin , this was sufficient to induce peak hemoglobin synthesis .
	manualset3
217362	1	420119	7	NULL	NULL	0	NULL	Addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of thiols to dithionite reduced microsomes resulted in relatively small spectral changes with maxima at 449 nm typical for ligand complexes of the ferrous cytochrome .
	manualset3
217363	2	420119	7	NULL	NULL	0	NULL	thiols	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of thiols to dithionite reduced microsomes resulted in relatively small spectral changes with maxima at 449 nm typical for ligand complexes of the ferrous cytochrome .
	manualset3
217364	3	420119	7	NULL	NULL	0	NULL	 dithionite reduced microsomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of thiols to dithionite reduced microsomes resulted in relatively small spectral changes with maxima at 449 nm typical for ligand complexes of the ferrous cytochrome .
	manualset3
217365	4	420119	7	NULL	NULL	0	NULL	small spectral changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of thiols to dithionite reduced microsomes resulted in relatively small spectral changes with maxima at 449 nm typical for ligand complexes of the ferrous cytochrome .
	manualset3
217366	5	420119	7	NULL	NULL	0	NULL	maxima	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of thiols to dithionite reduced microsomes resulted in relatively small spectral changes with maxima at 449 nm typical for ligand complexes of the ferrous cytochrome .
	manualset3
217367	6	420119	7	NULL	NULL	0	NULL	449 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of thiols to dithionite reduced microsomes resulted in relatively small spectral changes with maxima at 449 nm typical for ligand complexes of the ferrous cytochrome .
	manualset3
217368	7	420119	7	NULL	NULL	NULL	NULL	ligand complexes	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Addition of thiols to dithionite reduced microsomes resulted in relatively small spectral changes with maxima at 449 nm typical for ligand complexes of the ferrous cytochrome .
	manualset3
217369	8	420119	7	NULL	NULL	0	NULL	ferrous cytochrome	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Addition of thiols to dithionite reduced microsomes resulted in relatively small spectral changes with maxima at 449 nm typical for ligand complexes of the ferrous cytochrome .
	manualset3
217370	1	420120	7	NULL	NULL	0	NULL	Columns of cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Columns of cells were stimulated continuously or with trains of CRF pulses of varying pulse length ( 2-16 min ) , pulse period ( 20-160 min ) , and concentration , for 500 min .
	manualset3
217371	2	420120	7	NULL	NULL	0	NULL	 trains of CRF pulses	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Columns of cells were stimulated continuously or with trains of CRF pulses of varying pulse length ( 2-16 min ) , pulse period ( 20-160 min ) , and concentration , for 500 min .
	manualset3
217372	3	420120	7	NULL	NULL	0	NULL	varying pulse length	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Columns of cells were stimulated continuously or with trains of CRF pulses of varying pulse length ( 2-16 min ) , pulse period ( 20-160 min ) , and concentration , for 500 min .
	manualset3
217373	4	420120	7	NULL	NULL	0	NULL	2-16 min 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Columns of cells were stimulated continuously or with trains of CRF pulses of varying pulse length ( 2-16 min ) , pulse period ( 20-160 min ) , and concentration , for 500 min .
	manualset3
217374	5	420120	7	NULL	NULL	0	NULL	pulse period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Columns of cells were stimulated continuously or with trains of CRF pulses of varying pulse length ( 2-16 min ) , pulse period ( 20-160 min ) , and concentration , for 500 min .
	manualset3
217375	6	420120	7	NULL	NULL	0	NULL	20-160 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Columns of cells were stimulated continuously or with trains of CRF pulses of varying pulse length ( 2-16 min ) , pulse period ( 20-160 min ) , and concentration , for 500 min .
	manualset3
217376	7	420120	7	NULL	NULL	0	NULL	concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Columns of cells were stimulated continuously or with trains of CRF pulses of varying pulse length ( 2-16 min ) , pulse period ( 20-160 min ) , and concentration , for 500 min .
	manualset3
217377	8	420120	7	NULL	NULL	0	NULL	500 min	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Columns of cells were stimulated continuously or with trains of CRF pulses of varying pulse length ( 2-16 min ) , pulse period ( 20-160 min ) , and concentration , for 500 min .
	manualset3
217378	1	420121	7	NULL	NULL	0	NULL	military-unique curriculum	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The importance of a military-unique curriculum in active duty graduate medical education .
	manualset3
217379	2	420121	7	NULL	NULL	0	NULL	active duty graduate medical education	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The importance of a military-unique curriculum in active duty graduate medical education .
	manualset3
217380	1	420122	7	NULL	NULL	0	NULL	transcript	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the transcript of the fusion gene only contains the first 74 nucleotides of gene II mRNA , it is furthermore concluded that these nucleotides are already sufficient for gene V protein to exert its regulatory effect .
	manualset3
217381	2	420122	7	NULL	NULL	0	NULL	fusion gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the transcript of the fusion gene only contains the first 74 nucleotides of gene II mRNA , it is furthermore concluded that these nucleotides are already sufficient for gene V protein to exert its regulatory effect .
	manualset3
217382	3	420122	7	NULL	NULL	0	NULL	first 74 nucleotides 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the transcript of the fusion gene only contains the first 74 nucleotides of gene II mRNA , it is furthermore concluded that these nucleotides are already sufficient for gene V protein to exert its regulatory effect .
	manualset3
217383	4	420122	7	NULL	NULL	0	NULL	gene II mRNA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the transcript of the fusion gene only contains the first 74 nucleotides of gene II mRNA , it is furthermore concluded that these nucleotides are already sufficient for gene V protein to exert its regulatory effect .
	manualset3
217384	5	420122	7	NULL	NULL	0	NULL	nucleotides	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the transcript of the fusion gene only contains the first 74 nucleotides of gene II mRNA , it is furthermore concluded that these nucleotides are already sufficient for gene V protein to exert its regulatory effect .
	manualset3
217385	6	420122	7	NULL	NULL	0	NULL	gene V protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the transcript of the fusion gene only contains the first 74 nucleotides of gene II mRNA , it is furthermore concluded that these nucleotides are already sufficient for gene V protein to exert its regulatory effect .
	manualset3
217386	7	420122	7	NULL	NULL	0	NULL	regulatory effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Since the transcript of the fusion gene only contains the first 74 nucleotides of gene II mRNA , it is furthermore concluded that these nucleotides are already sufficient for gene V protein to exert its regulatory effect .
	manualset3
217387	1	420123	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of serological properties , specificity and the range of action has revealed affinity between Y. pseudotuberculosis phages ( PST , 3M , Kotlyarova , 2344 , 2391 ) , some coliphages ( T2 , T3 , T4 ) and Sh .
	manualset3
217388	2	420123	7	NULL	NULL	0	NULL	serological properties	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of serological properties , specificity and the range of action has revealed affinity between Y. pseudotuberculosis phages ( PST , 3M , Kotlyarova , 2344 , 2391 ) , some coliphages ( T2 , T3 , T4 ) and Sh .
	manualset3
217389	3	420123	7	NULL	NULL	0	NULL	specificity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of serological properties , specificity and the range of action has revealed affinity between Y. pseudotuberculosis phages ( PST , 3M , Kotlyarova , 2344 , 2391 ) , some coliphages ( T2 , T3 , T4 ) and Sh .
	manualset3
217390	4	420123	7	NULL	NULL	0	NULL	 range of action 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of serological properties , specificity and the range of action has revealed affinity between Y. pseudotuberculosis phages ( PST , 3M , Kotlyarova , 2344 , 2391 ) , some coliphages ( T2 , T3 , T4 ) and Sh .
	manualset3
217391	5	420123	7	NULL	NULL	0	NULL	affinity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of serological properties , specificity and the range of action has revealed affinity between Y. pseudotuberculosis phages ( PST , 3M , Kotlyarova , 2344 , 2391 ) , some coliphages ( T2 , T3 , T4 ) and Sh .
	manualset3
217392	6	420123	7	NULL	NULL	0	NULL	Y. pseudotuberculosis phages	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of serological properties , specificity and the range of action has revealed affinity between Y. pseudotuberculosis phages ( PST , 3M , Kotlyarova , 2344 , 2391 ) , some coliphages ( T2 , T3 , T4 ) and Sh .
	manualset3
217393	7	420123	7	NULL	NULL	0	NULL	PST	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of serological properties , specificity and the range of action has revealed affinity between Y. pseudotuberculosis phages ( PST , 3M , Kotlyarova , 2344 , 2391 ) , some coliphages ( T2 , T3 , T4 ) and Sh .
	manualset3
217394	8	420123	7	NULL	NULL	0	NULL	3M	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of serological properties , specificity and the range of action has revealed affinity between Y. pseudotuberculosis phages ( PST , 3M , Kotlyarova , 2344 , 2391 ) , some coliphages ( T2 , T3 , T4 ) and Sh .
	manualset3
217395	9	420123	7	NULL	NULL	0	NULL	Kotlyarova	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of serological properties , specificity and the range of action has revealed affinity between Y. pseudotuberculosis phages ( PST , 3M , Kotlyarova , 2344 , 2391 ) , some coliphages ( T2 , T3 , T4 ) and Sh .
	manualset3
217396	10	420123	7	NULL	NULL	0	NULL	2344 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of serological properties , specificity and the range of action has revealed affinity between Y. pseudotuberculosis phages ( PST , 3M , Kotlyarova , 2344 , 2391 ) , some coliphages ( T2 , T3 , T4 ) and Sh .
	manualset3
217397	11	420123	7	NULL	NULL	0	NULL	2391	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of serological properties , specificity and the range of action has revealed affinity between Y. pseudotuberculosis phages ( PST , 3M , Kotlyarova , 2344 , 2391 ) , some coliphages ( T2 , T3 , T4 ) and Sh .
	manualset3
217398	12	420123	7	NULL	NULL	0	NULL	coliphages	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of serological properties , specificity and the range of action has revealed affinity between Y. pseudotuberculosis phages ( PST , 3M , Kotlyarova , 2344 , 2391 ) , some coliphages ( T2 , T3 , T4 ) and Sh .
	manualset3
217399	13	420123	7	NULL	NULL	0	NULL	T2	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of serological properties , specificity and the range of action has revealed affinity between Y. pseudotuberculosis phages ( PST , 3M , Kotlyarova , 2344 , 2391 ) , some coliphages ( T2 , T3 , T4 ) and Sh .
	manualset3
217400	14	420123	7	NULL	NULL	0	NULL	T3	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of serological properties , specificity and the range of action has revealed affinity between Y. pseudotuberculosis phages ( PST , 3M , Kotlyarova , 2344 , 2391 ) , some coliphages ( T2 , T3 , T4 ) and Sh .
	manualset3
217401	15	420123	7	NULL	NULL	0	NULL	T4	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of serological properties , specificity and the range of action has revealed affinity between Y. pseudotuberculosis phages ( PST , 3M , Kotlyarova , 2344 , 2391 ) , some coliphages ( T2 , T3 , T4 ) and Sh .
	manualset3
217402	16	420123	7	NULL	NULL	0	NULL	Sh	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of serological properties , specificity and the range of action has revealed affinity between Y. pseudotuberculosis phages ( PST , 3M , Kotlyarova , 2344 , 2391 ) , some coliphages ( T2 , T3 , T4 ) and Sh .
	manualset3
217403	1	420124	7	NULL	NULL	0	NULL	CA 15.3 sensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	CA 15.3 sensitivity at diagnosis ( 60 % ) and for detecting relapse ( 44 % ) was lower than that of CA 125 ( 90 % and 64.7 % , respectively ) .
	manualset3
217404	2	420124	7	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	CA 15.3 sensitivity at diagnosis ( 60 % ) and for detecting relapse ( 44 % ) was lower than that of CA 125 ( 90 % and 64.7 % , respectively ) .
	manualset3
217405	3	420124	7	NULL	NULL	0	NULL	60 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	CA 15.3 sensitivity at diagnosis ( 60 % ) and for detecting relapse ( 44 % ) was lower than that of CA 125 ( 90 % and 64.7 % , respectively ) .
	manualset3
217406	4	420124	7	NULL	NULL	0	NULL	relapse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	CA 15.3 sensitivity at diagnosis ( 60 % ) and for detecting relapse ( 44 % ) was lower than that of CA 125 ( 90 % and 64.7 % , respectively ) .
	manualset3
217407	5	420124	7	NULL	NULL	0	NULL	44 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	CA 15.3 sensitivity at diagnosis ( 60 % ) and for detecting relapse ( 44 % ) was lower than that of CA 125 ( 90 % and 64.7 % , respectively ) .
	manualset3
217408	6	420124	7	NULL	NULL	0	NULL	CA 125	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	CA 15.3 sensitivity at diagnosis ( 60 % ) and for detecting relapse ( 44 % ) was lower than that of CA 125 ( 90 % and 64.7 % , respectively ) .
	manualset3
217409	7	420124	7	NULL	NULL	0	NULL	 90 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	CA 15.3 sensitivity at diagnosis ( 60 % ) and for detecting relapse ( 44 % ) was lower than that of CA 125 ( 90 % and 64.7 % , respectively ) .
	manualset3
217410	8	420124	7	NULL	NULL	0	NULL	64.7 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	CA 15.3 sensitivity at diagnosis ( 60 % ) and for detecting relapse ( 44 % ) was lower than that of CA 125 ( 90 % and 64.7 % , respectively ) .
	manualset3
217411	1	420125	7	NULL	NULL	0	NULL	TCD 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that TCD is highly specific in detecting both ACA and PCA vasospasm on arteries that can be insonated .
	manualset3
217412	2	420125	7	NULL	NULL	0	NULL	ACA vasospasm	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that TCD is highly specific in detecting both ACA and PCA vasospasm on arteries that can be insonated .
	manualset3
217413	3	420125	7	NULL	NULL	0	NULL	PCA vasospasm 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that TCD is highly specific in detecting both ACA and PCA vasospasm on arteries that can be insonated .
	manualset3
217414	4	420125	7	NULL	NULL	0	NULL	arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that TCD is highly specific in detecting both ACA and PCA vasospasm on arteries that can be insonated .
	manualset3
217415	1	420126	7	NULL	NULL	0	NULL	Household-weight latex gloves	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Household-weight latex gloves were protective against CHC allergy .
	manualset3
217416	2	420126	7	NULL	NULL	0	NULL	CHC allergy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Household-weight latex gloves were protective against CHC allergy .
	manualset3
217417	1	420127	7	NULL	NULL	0	NULL	 mini-systems	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	We propose that in order to comprehend how these mini-systems integrate to facilitate uterine contraction during labor ( preterm or term ) we must , in concert with biological experimentation , construct detailed mathematical descriptions of our findings .
	manualset3
217418	2	420127	7	NULL	NULL	0	NULL	uterine contraction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We propose that in order to comprehend how these mini-systems integrate to facilitate uterine contraction during labor ( preterm or term ) we must , in concert with biological experimentation , construct detailed mathematical descriptions of our findings .
	manualset3
217419	3	420127	7	NULL	NULL	0	NULL	labor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We propose that in order to comprehend how these mini-systems integrate to facilitate uterine contraction during labor ( preterm or term ) we must , in concert with biological experimentation , construct detailed mathematical descriptions of our findings .
	manualset3
217420	4	420127	7	NULL	NULL	0	NULL	preterm 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	We propose that in order to comprehend how these mini-systems integrate to facilitate uterine contraction during labor ( preterm or term ) we must , in concert with biological experimentation , construct detailed mathematical descriptions of our findings .
	manualset3
217421	5	420127	7	NULL	NULL	0	NULL	term	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	We propose that in order to comprehend how these mini-systems integrate to facilitate uterine contraction during labor ( preterm or term ) we must , in concert with biological experimentation , construct detailed mathematical descriptions of our findings .
	manualset3
217422	6	420127	7	NULL	NULL	0	NULL	biological experimentation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We propose that in order to comprehend how these mini-systems integrate to facilitate uterine contraction during labor ( preterm or term ) we must , in concert with biological experimentation , construct detailed mathematical descriptions of our findings .
	manualset3
217423	7	420127	7	NULL	NULL	0	NULL	construct	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We propose that in order to comprehend how these mini-systems integrate to facilitate uterine contraction during labor ( preterm or term ) we must , in concert with biological experimentation , construct detailed mathematical descriptions of our findings .
	manualset3
217424	8	420127	7	NULL	NULL	0	NULL	mathematical descriptions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We propose that in order to comprehend how these mini-systems integrate to facilitate uterine contraction during labor ( preterm or term ) we must , in concert with biological experimentation , construct detailed mathematical descriptions of our findings .
	manualset3
217425	9	420127	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We propose that in order to comprehend how these mini-systems integrate to facilitate uterine contraction during labor ( preterm or term ) we must , in concert with biological experimentation , construct detailed mathematical descriptions of our findings .
	manualset3
217426	1	420128	7	NULL	NULL	0	NULL	R gene families	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , similar to that for many R gene families , several RGA loci were found in clusters , suggesting their potential evolutionary relationship with R genes .
	manualset3
217427	2	420128	7	NULL	NULL	0	NULL	RGA loci	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , similar to that for many R gene families , several RGA loci were found in clusters , suggesting their potential evolutionary relationship with R genes .
	manualset3
217428	3	420128	7	NULL	NULL	0	NULL	clusters	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , similar to that for many R gene families , several RGA loci were found in clusters , suggesting their potential evolutionary relationship with R genes .
	manualset3
217429	4	420128	7	NULL	NULL	NULL	NULL	potential evolutionary relationship	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Furthermore , similar to that for many R gene families , several RGA loci were found in clusters , suggesting their potential evolutionary relationship with R genes .
	manualset3
217430	5	420128	7	NULL	NULL	0	NULL	R genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , similar to that for many R gene families , several RGA loci were found in clusters , suggesting their potential evolutionary relationship with R genes .
	manualset3
217431	1	420129	7	NULL	NULL	0	NULL	Effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of Bromhexine on the phospholipid content of rabbit lungs ) .
	manualset3
217432	2	420129	7	NULL	NULL	0	NULL	Bromhexine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of Bromhexine on the phospholipid content of rabbit lungs ) .
	manualset3
217433	3	420129	7	NULL	NULL	0	NULL	phospholipid content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of Bromhexine on the phospholipid content of rabbit lungs ) .
	manualset3
217434	4	420129	7	NULL	NULL	0	NULL	rabbit lungs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of Bromhexine on the phospholipid content of rabbit lungs ) .
	manualset3
217435	1	420130	7	NULL	NULL	0	NULL	 schizophrenia research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous schizophrenia research suggests poor cognitive control is associated with schizophrenia speech symptoms .
	manualset3
217436	2	420130	7	NULL	NULL	0	NULL	poor cognitive control	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous schizophrenia research suggests poor cognitive control is associated with schizophrenia speech symptoms .
	manualset3
217437	3	420130	7	NULL	NULL	0	NULL	schizophrenia speech symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous schizophrenia research suggests poor cognitive control is associated with schizophrenia speech symptoms .
	manualset3
217444	1	420131	7	NULL	NULL	0	NULL	Seven	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven had final IOP readings less than or equal to 25 mmHg ( 63.6 % ) .
	manualset3
217445	2	420131	7	NULL	NULL	0	NULL	 final IOP readings	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven had final IOP readings less than or equal to 25 mmHg ( 63.6 % ) .
	manualset3
217446	3	420131	7	NULL	NULL	0	NULL	25 mmHg	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven had final IOP readings less than or equal to 25 mmHg ( 63.6 % ) .
	manualset3
217447	4	420131	7	NULL	NULL	0	NULL	63.6 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven had final IOP readings less than or equal to 25 mmHg ( 63.6 % ) .
	manualset3
217448	1	420132	7	NULL	NULL	0	NULL	retinoblastoma protein ( Rb )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the retinoblastoma protein ( Rb ) functions as a checkpoint in the cell cycle , it also regulates differentiation .
	manualset3
217449	2	420132	7	NULL	NULL	0	NULL	checkpoint	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the retinoblastoma protein ( Rb ) functions as a checkpoint in the cell cycle , it also regulates differentiation .
	manualset3
217450	3	420132	7	NULL	NULL	0	NULL	cell cycle	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the retinoblastoma protein ( Rb ) functions as a checkpoint in the cell cycle , it also regulates differentiation .
	manualset3
217451	4	420132	7	NULL	NULL	0	NULL	differentiation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the retinoblastoma protein ( Rb ) functions as a checkpoint in the cell cycle , it also regulates differentiation .
	manualset3
217452	1	420133	7	NULL	NULL	0	NULL	Hip ganglion cyst	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hip ganglion cyst associated with developmental dysplasia of hip in a child-a case report .
	manualset3
217453	2	420133	7	NULL	NULL	0	NULL	developmental dysplasia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hip ganglion cyst associated with developmental dysplasia of hip in a child-a case report .
	manualset3
217454	3	420133	7	NULL	NULL	0	NULL	hip	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Hip ganglion cyst associated with developmental dysplasia of hip in a child-a case report .
	manualset3
217455	4	420133	7	NULL	NULL	0	NULL	child-a case report 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Hip ganglion cyst associated with developmental dysplasia of hip in a child-a case report .
	manualset3
217456	1	420134	7	NULL	NULL	NULL	NULL	origin	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On the origin and early use of the term vicarious trial and error ( VTE ) .
	manualset3
217457	2	420134	7	NULL	NULL	0	NULL	early use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the origin and early use of the term vicarious trial and error ( VTE ) .
	manualset3
217458	3	420134	7	NULL	NULL	0	NULL	vicarious trial and error ( VTE )	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the origin and early use of the term vicarious trial and error ( VTE ) .
	manualset3
218831	4	420134	7	NULL	NULL	0	NULL	term	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the origin and early use of the term vicarious trial and error ( VTE ) .
	manualset3
217459	1	420135	7	NULL	NULL	0	NULL	Linear IgA dermatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Linear IgA dermatitis was diagnosed in a 13-year old girl with erythema annulare centrifugum ( EAC ) on the basis of the criteria laid down by Jablonska : vesiculo-bullous eruption with specific patterns on subsequent flare-ups , subepidermal vesicles and bullae with papillary eosinophilic abscesses in erythematous areas , positive linear IgA antibody response at direct immunofluorescence in the lamina basal , absence of intolerance to gluten and responsiveness to sulfapyridine and dapsone .
	manualset3
217460	2	420135	7	NULL	NULL	0	NULL	13-year old girl	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Linear IgA dermatitis was diagnosed in a 13-year old girl with erythema annulare centrifugum ( EAC ) on the basis of the criteria laid down by Jablonska : vesiculo-bullous eruption with specific patterns on subsequent flare-ups , subepidermal vesicles and bullae with papillary eosinophilic abscesses in erythematous areas , positive linear IgA antibody response at direct immunofluorescence in the lamina basal , absence of intolerance to gluten and responsiveness to sulfapyridine and dapsone .
	manualset3
217461	3	420135	7	NULL	NULL	NULL	NULL	erythema annulare centrifugum ( EAC )	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Linear IgA dermatitis was diagnosed in a 13-year old girl with erythema annulare centrifugum ( EAC ) on the basis of the criteria laid down by Jablonska : vesiculo-bullous eruption with specific patterns on subsequent flare-ups , subepidermal vesicles and bullae with papillary eosinophilic abscesses in erythematous areas , positive linear IgA antibody response at direct immunofluorescence in the lamina basal , absence of intolerance to gluten and responsiveness to sulfapyridine and dapsone .
	manualset3
217462	4	420135	7	NULL	NULL	0	NULL	basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Linear IgA dermatitis was diagnosed in a 13-year old girl with erythema annulare centrifugum ( EAC ) on the basis of the criteria laid down by Jablonska : vesiculo-bullous eruption with specific patterns on subsequent flare-ups , subepidermal vesicles and bullae with papillary eosinophilic abscesses in erythematous areas , positive linear IgA antibody response at direct immunofluorescence in the lamina basal , absence of intolerance to gluten and responsiveness to sulfapyridine and dapsone .
	manualset3
217463	5	420135	7	NULL	NULL	0	NULL	criteria	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Linear IgA dermatitis was diagnosed in a 13-year old girl with erythema annulare centrifugum ( EAC ) on the basis of the criteria laid down by Jablonska : vesiculo-bullous eruption with specific patterns on subsequent flare-ups , subepidermal vesicles and bullae with papillary eosinophilic abscesses in erythematous areas , positive linear IgA antibody response at direct immunofluorescence in the lamina basal , absence of intolerance to gluten and responsiveness to sulfapyridine and dapsone .
	manualset3
217464	6	420135	7	NULL	NULL	0	NULL	Jablonska : vesiculo-bullous eruption	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Linear IgA dermatitis was diagnosed in a 13-year old girl with erythema annulare centrifugum ( EAC ) on the basis of the criteria laid down by Jablonska : vesiculo-bullous eruption with specific patterns on subsequent flare-ups , subepidermal vesicles and bullae with papillary eosinophilic abscesses in erythematous areas , positive linear IgA antibody response at direct immunofluorescence in the lamina basal , absence of intolerance to gluten and responsiveness to sulfapyridine and dapsone .
	manualset3
217465	7	420135	7	NULL	NULL	0	NULL	specific patterns	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Linear IgA dermatitis was diagnosed in a 13-year old girl with erythema annulare centrifugum ( EAC ) on the basis of the criteria laid down by Jablonska : vesiculo-bullous eruption with specific patterns on subsequent flare-ups , subepidermal vesicles and bullae with papillary eosinophilic abscesses in erythematous areas , positive linear IgA antibody response at direct immunofluorescence in the lamina basal , absence of intolerance to gluten and responsiveness to sulfapyridine and dapsone .
	manualset3
217466	8	420135	7	NULL	NULL	0	NULL	subsequent flare-ups	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Linear IgA dermatitis was diagnosed in a 13-year old girl with erythema annulare centrifugum ( EAC ) on the basis of the criteria laid down by Jablonska : vesiculo-bullous eruption with specific patterns on subsequent flare-ups , subepidermal vesicles and bullae with papillary eosinophilic abscesses in erythematous areas , positive linear IgA antibody response at direct immunofluorescence in the lamina basal , absence of intolerance to gluten and responsiveness to sulfapyridine and dapsone .
	manualset3
217467	9	420135	7	NULL	NULL	0	NULL	subepidermal vesicles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Linear IgA dermatitis was diagnosed in a 13-year old girl with erythema annulare centrifugum ( EAC ) on the basis of the criteria laid down by Jablonska : vesiculo-bullous eruption with specific patterns on subsequent flare-ups , subepidermal vesicles and bullae with papillary eosinophilic abscesses in erythematous areas , positive linear IgA antibody response at direct immunofluorescence in the lamina basal , absence of intolerance to gluten and responsiveness to sulfapyridine and dapsone .
	manualset3
217468	10	420135	7	NULL	NULL	0	NULL	bullae with papillary eosinophilic abscesses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Linear IgA dermatitis was diagnosed in a 13-year old girl with erythema annulare centrifugum ( EAC ) on the basis of the criteria laid down by Jablonska : vesiculo-bullous eruption with specific patterns on subsequent flare-ups , subepidermal vesicles and bullae with papillary eosinophilic abscesses in erythematous areas , positive linear IgA antibody response at direct immunofluorescence in the lamina basal , absence of intolerance to gluten and responsiveness to sulfapyridine and dapsone .
	manualset3
217469	11	420135	7	NULL	NULL	NULL	NULL	erythematous areas	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Linear IgA dermatitis was diagnosed in a 13-year old girl with erythema annulare centrifugum ( EAC ) on the basis of the criteria laid down by Jablonska : vesiculo-bullous eruption with specific patterns on subsequent flare-ups , subepidermal vesicles and bullae with papillary eosinophilic abscesses in erythematous areas , positive linear IgA antibody response at direct immunofluorescence in the lamina basal , absence of intolerance to gluten and responsiveness to sulfapyridine and dapsone .
	manualset3
217470	12	420135	7	NULL	NULL	0	NULL	positive linear IgA antibody response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Linear IgA dermatitis was diagnosed in a 13-year old girl with erythema annulare centrifugum ( EAC ) on the basis of the criteria laid down by Jablonska : vesiculo-bullous eruption with specific patterns on subsequent flare-ups , subepidermal vesicles and bullae with papillary eosinophilic abscesses in erythematous areas , positive linear IgA antibody response at direct immunofluorescence in the lamina basal , absence of intolerance to gluten and responsiveness to sulfapyridine and dapsone .
	manualset3
217471	13	420135	7	NULL	NULL	0	NULL	direct immunofluorescence	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Linear IgA dermatitis was diagnosed in a 13-year old girl with erythema annulare centrifugum ( EAC ) on the basis of the criteria laid down by Jablonska : vesiculo-bullous eruption with specific patterns on subsequent flare-ups , subepidermal vesicles and bullae with papillary eosinophilic abscesses in erythematous areas , positive linear IgA antibody response at direct immunofluorescence in the lamina basal , absence of intolerance to gluten and responsiveness to sulfapyridine and dapsone .
	manualset3
217472	14	420135	7	NULL	NULL	0	NULL	lamina basal 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Linear IgA dermatitis was diagnosed in a 13-year old girl with erythema annulare centrifugum ( EAC ) on the basis of the criteria laid down by Jablonska : vesiculo-bullous eruption with specific patterns on subsequent flare-ups , subepidermal vesicles and bullae with papillary eosinophilic abscesses in erythematous areas , positive linear IgA antibody response at direct immunofluorescence in the lamina basal , absence of intolerance to gluten and responsiveness to sulfapyridine and dapsone .
	manualset3
217473	15	420135	7	NULL	NULL	0	NULL	 intolerance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Linear IgA dermatitis was diagnosed in a 13-year old girl with erythema annulare centrifugum ( EAC ) on the basis of the criteria laid down by Jablonska : vesiculo-bullous eruption with specific patterns on subsequent flare-ups , subepidermal vesicles and bullae with papillary eosinophilic abscesses in erythematous areas , positive linear IgA antibody response at direct immunofluorescence in the lamina basal , absence of intolerance to gluten and responsiveness to sulfapyridine and dapsone .
	manualset3
217474	16	420135	7	NULL	NULL	0	NULL	gluten	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Linear IgA dermatitis was diagnosed in a 13-year old girl with erythema annulare centrifugum ( EAC ) on the basis of the criteria laid down by Jablonska : vesiculo-bullous eruption with specific patterns on subsequent flare-ups , subepidermal vesicles and bullae with papillary eosinophilic abscesses in erythematous areas , positive linear IgA antibody response at direct immunofluorescence in the lamina basal , absence of intolerance to gluten and responsiveness to sulfapyridine and dapsone .
	manualset3
217475	17	420135	7	NULL	NULL	0	NULL	responsiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Linear IgA dermatitis was diagnosed in a 13-year old girl with erythema annulare centrifugum ( EAC ) on the basis of the criteria laid down by Jablonska : vesiculo-bullous eruption with specific patterns on subsequent flare-ups , subepidermal vesicles and bullae with papillary eosinophilic abscesses in erythematous areas , positive linear IgA antibody response at direct immunofluorescence in the lamina basal , absence of intolerance to gluten and responsiveness to sulfapyridine and dapsone .
	manualset3
217476	18	420135	7	NULL	NULL	0	NULL	sulfapyridine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Linear IgA dermatitis was diagnosed in a 13-year old girl with erythema annulare centrifugum ( EAC ) on the basis of the criteria laid down by Jablonska : vesiculo-bullous eruption with specific patterns on subsequent flare-ups , subepidermal vesicles and bullae with papillary eosinophilic abscesses in erythematous areas , positive linear IgA antibody response at direct immunofluorescence in the lamina basal , absence of intolerance to gluten and responsiveness to sulfapyridine and dapsone .
	manualset3
217477	19	420135	7	NULL	NULL	0	NULL	dapsone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Linear IgA dermatitis was diagnosed in a 13-year old girl with erythema annulare centrifugum ( EAC ) on the basis of the criteria laid down by Jablonska : vesiculo-bullous eruption with specific patterns on subsequent flare-ups , subepidermal vesicles and bullae with papillary eosinophilic abscesses in erythematous areas , positive linear IgA antibody response at direct immunofluorescence in the lamina basal , absence of intolerance to gluten and responsiveness to sulfapyridine and dapsone .
	manualset3
217478	1	420136	7	NULL	NULL	0	NULL	Flow cytometry 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Flow cytometry was used to determine platelet-monocyte complexes ( PMC ) , platelet-neutrophil complexes ( PNC ) , basal and adenosine diphosphate ( ADP ) - stimulated platelet CD62P expression .
	manualset3
217479	2	420136	7	NULL	NULL	0	NULL	platelet-monocyte complexes ( PMC )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Flow cytometry was used to determine platelet-monocyte complexes ( PMC ) , platelet-neutrophil complexes ( PNC ) , basal and adenosine diphosphate ( ADP ) - stimulated platelet CD62P expression .
	manualset3
217480	3	420136	7	NULL	NULL	0	NULL	 platelet-neutrophil complexes ( PNC )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Flow cytometry was used to determine platelet-monocyte complexes ( PMC ) , platelet-neutrophil complexes ( PNC ) , basal and adenosine diphosphate ( ADP ) - stimulated platelet CD62P expression .
	manualset3
217481	4	420136	7	NULL	NULL	0	NULL	basal and adenosine diphosphate ( ADP ) - stimulated platelet CD62P expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Flow cytometry was used to determine platelet-monocyte complexes ( PMC ) , platelet-neutrophil complexes ( PNC ) , basal and adenosine diphosphate ( ADP ) - stimulated platelet CD62P expression .
	manualset3
217482	1	420137	7	NULL	NULL	0	NULL	Early detection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Early detection and intervention is essential for cure .
	manualset3
217483	2	420137	7	NULL	NULL	NULL	NULL	 intervention	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early detection and intervention is essential for cure .
	manualset3
217484	3	420137	7	NULL	NULL	0	NULL	cure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Early detection and intervention is essential for cure .
	manualset3
217485	1	420138	7	NULL	NULL	0	NULL	 issues	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To address these issues , we have taken advantage of a mouse mAb , coined C355 .1 , and studied its reactivity against a panel of liver tissue from normal subjects as well as a panel of liver specimens from patients with PBC , progressive sclerosing cholangitis , and chronic active hepatitis ( CAH ) .
	manualset3
217486	2	420138	7	NULL	NULL	0	NULL	advantage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To address these issues , we have taken advantage of a mouse mAb , coined C355 .1 , and studied its reactivity against a panel of liver tissue from normal subjects as well as a panel of liver specimens from patients with PBC , progressive sclerosing cholangitis , and chronic active hepatitis ( CAH ) .
	manualset3
217487	3	420138	7	NULL	NULL	0	NULL	mouse mAb	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To address these issues , we have taken advantage of a mouse mAb , coined C355 .1 , and studied its reactivity against a panel of liver tissue from normal subjects as well as a panel of liver specimens from patients with PBC , progressive sclerosing cholangitis , and chronic active hepatitis ( CAH ) .
	manualset3
217488	4	420138	7	NULL	NULL	0	NULL	C355 .1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To address these issues , we have taken advantage of a mouse mAb , coined C355 .1 , and studied its reactivity against a panel of liver tissue from normal subjects as well as a panel of liver specimens from patients with PBC , progressive sclerosing cholangitis , and chronic active hepatitis ( CAH ) .
	manualset3
217489	5	420138	7	NULL	NULL	0	NULL	 reactivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To address these issues , we have taken advantage of a mouse mAb , coined C355 .1 , and studied its reactivity against a panel of liver tissue from normal subjects as well as a panel of liver specimens from patients with PBC , progressive sclerosing cholangitis , and chronic active hepatitis ( CAH ) .
	manualset3
217490	6	420138	7	NULL	NULL	0	NULL	panel of liver tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	To address these issues , we have taken advantage of a mouse mAb , coined C355 .1 , and studied its reactivity against a panel of liver tissue from normal subjects as well as a panel of liver specimens from patients with PBC , progressive sclerosing cholangitis , and chronic active hepatitis ( CAH ) .
	manualset3
217491	7	420138	7	NULL	NULL	0	NULL	normal subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To address these issues , we have taken advantage of a mouse mAb , coined C355 .1 , and studied its reactivity against a panel of liver tissue from normal subjects as well as a panel of liver specimens from patients with PBC , progressive sclerosing cholangitis , and chronic active hepatitis ( CAH ) .
	manualset3
217492	8	420138	7	NULL	NULL	0	NULL	panel of liver specimens	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	To address these issues , we have taken advantage of a mouse mAb , coined C355 .1 , and studied its reactivity against a panel of liver tissue from normal subjects as well as a panel of liver specimens from patients with PBC , progressive sclerosing cholangitis , and chronic active hepatitis ( CAH ) .
	manualset3
217493	9	420138	7	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To address these issues , we have taken advantage of a mouse mAb , coined C355 .1 , and studied its reactivity against a panel of liver tissue from normal subjects as well as a panel of liver specimens from patients with PBC , progressive sclerosing cholangitis , and chronic active hepatitis ( CAH ) .
	manualset3
217494	10	420138	7	NULL	NULL	0	NULL	PBC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To address these issues , we have taken advantage of a mouse mAb , coined C355 .1 , and studied its reactivity against a panel of liver tissue from normal subjects as well as a panel of liver specimens from patients with PBC , progressive sclerosing cholangitis , and chronic active hepatitis ( CAH ) .
	manualset3
217495	11	420138	7	NULL	NULL	0	NULL	progressive sclerosing cholangitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To address these issues , we have taken advantage of a mouse mAb , coined C355 .1 , and studied its reactivity against a panel of liver tissue from normal subjects as well as a panel of liver specimens from patients with PBC , progressive sclerosing cholangitis , and chronic active hepatitis ( CAH ) .
	manualset3
217496	12	420138	7	NULL	NULL	0	NULL	chronic active hepatitis ( CAH )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	To address these issues , we have taken advantage of a mouse mAb , coined C355 .1 , and studied its reactivity against a panel of liver tissue from normal subjects as well as a panel of liver specimens from patients with PBC , progressive sclerosing cholangitis , and chronic active hepatitis ( CAH ) .
	manualset3
217497	1	420139	7	NULL	NULL	0	NULL	organs cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We have used organs cultures of murine mesentery as a model system to investigate the mechanisms by which B16-F10 melanoma cells invade normal tissues .
	manualset3
217498	2	420139	7	NULL	NULL	0	NULL	murine mesentery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We have used organs cultures of murine mesentery as a model system to investigate the mechanisms by which B16-F10 melanoma cells invade normal tissues .
	manualset3
217499	3	420139	7	NULL	NULL	0	NULL	model system	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We have used organs cultures of murine mesentery as a model system to investigate the mechanisms by which B16-F10 melanoma cells invade normal tissues .
	manualset3
217500	4	420139	7	NULL	NULL	0	NULL	mechanisms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We have used organs cultures of murine mesentery as a model system to investigate the mechanisms by which B16-F10 melanoma cells invade normal tissues .
	manualset3
217501	5	420139	7	NULL	NULL	0	NULL	B16-F10 melanoma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We have used organs cultures of murine mesentery as a model system to investigate the mechanisms by which B16-F10 melanoma cells invade normal tissues .
	manualset3
217502	6	420139	7	NULL	NULL	0	NULL	normal tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	We have used organs cultures of murine mesentery as a model system to investigate the mechanisms by which B16-F10 melanoma cells invade normal tissues .
	manualset3
217503	1	420140	7	NULL	NULL	0	NULL	( C5Me5 ) 3Y	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolated ( C5Me5 ) 3Y was found to metalate benzene and toluene with concomitant formation of C5Me5H , a reaction contrary to the normal pKa values of these hydrocarbons .
	manualset3
217504	2	420140	7	NULL	NULL	0	NULL	 benzene 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolated ( C5Me5 ) 3Y was found to metalate benzene and toluene with concomitant formation of C5Me5H , a reaction contrary to the normal pKa values of these hydrocarbons .
	manualset3
217505	3	420140	7	NULL	NULL	0	NULL	toluene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolated ( C5Me5 ) 3Y was found to metalate benzene and toluene with concomitant formation of C5Me5H , a reaction contrary to the normal pKa values of these hydrocarbons .
	manualset3
217506	4	420140	7	NULL	NULL	0	NULL	concomitant formation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolated ( C5Me5 ) 3Y was found to metalate benzene and toluene with concomitant formation of C5Me5H , a reaction contrary to the normal pKa values of these hydrocarbons .
	manualset3
217507	5	420140	7	NULL	NULL	0	NULL	C5Me5H	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolated ( C5Me5 ) 3Y was found to metalate benzene and toluene with concomitant formation of C5Me5H , a reaction contrary to the normal pKa values of these hydrocarbons .
	manualset3
217508	6	420140	7	NULL	NULL	0	NULL	 reaction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolated ( C5Me5 ) 3Y was found to metalate benzene and toluene with concomitant formation of C5Me5H , a reaction contrary to the normal pKa values of these hydrocarbons .
	manualset3
217509	7	420140	7	NULL	NULL	0	NULL	normal pKa values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolated ( C5Me5 ) 3Y was found to metalate benzene and toluene with concomitant formation of C5Me5H , a reaction contrary to the normal pKa values of these hydrocarbons .
	manualset3
217510	8	420140	7	NULL	NULL	0	NULL	hydrocarbons	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolated ( C5Me5 ) 3Y was found to metalate benzene and toluene with concomitant formation of C5Me5H , a reaction contrary to the normal pKa values of these hydrocarbons .
	manualset3
217512	1	420141	7	NULL	NULL	NULL	NULL	effect 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We study this effect on an example of a stochastic birth-death process with rates modulated by a colored ( that is , correlated ) Gaussian noise .
	manualset3
217513	2	420141	7	NULL	NULL	NULL	NULL	example	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We study this effect on an example of a stochastic birth-death process with rates modulated by a colored ( that is , correlated ) Gaussian noise .
	manualset3
217514	3	420141	7	NULL	NULL	NULL	NULL	stochastic birth-death process	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We study this effect on an example of a stochastic birth-death process with rates modulated by a colored ( that is , correlated ) Gaussian noise .
	manualset3
217515	5	420141	7	NULL	NULL	0	NULL	colored Gaussian noise	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We study this effect on an example of a stochastic birth-death process with rates modulated by a colored ( that is , correlated ) Gaussian noise .
	manualset3
217516	4	420141	7	NULL	NULL	0	NULL	 rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We study this effect on an example of a stochastic birth-death process with rates modulated by a colored ( that is , correlated ) Gaussian noise .
	manualset3
217517	1	420142	7	NULL	NULL	0	NULL	 U1A 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , U1A represents a novel class of protein which shuttles between cytoplasm and nucleus and whose intracellular distribution can be altered by the number of free binding sites for the protein present in the cytoplasm or the nucleus .
	manualset3
217518	2	420142	7	NULL	NULL	0	NULL	novel class	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , U1A represents a novel class of protein which shuttles between cytoplasm and nucleus and whose intracellular distribution can be altered by the number of free binding sites for the protein present in the cytoplasm or the nucleus .
	manualset3
217519	3	420142	7	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , U1A represents a novel class of protein which shuttles between cytoplasm and nucleus and whose intracellular distribution can be altered by the number of free binding sites for the protein present in the cytoplasm or the nucleus .
	manualset3
217520	4	420142	7	NULL	NULL	0	NULL	cytoplasm	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , U1A represents a novel class of protein which shuttles between cytoplasm and nucleus and whose intracellular distribution can be altered by the number of free binding sites for the protein present in the cytoplasm or the nucleus .
	manualset3
217521	5	420142	7	NULL	NULL	0	NULL	nucleus 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , U1A represents a novel class of protein which shuttles between cytoplasm and nucleus and whose intracellular distribution can be altered by the number of free binding sites for the protein present in the cytoplasm or the nucleus .
	manualset3
217522	6	420142	7	NULL	NULL	0	NULL	intracellular distribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , U1A represents a novel class of protein which shuttles between cytoplasm and nucleus and whose intracellular distribution can be altered by the number of free binding sites for the protein present in the cytoplasm or the nucleus .
	manualset3
217523	7	420142	7	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , U1A represents a novel class of protein which shuttles between cytoplasm and nucleus and whose intracellular distribution can be altered by the number of free binding sites for the protein present in the cytoplasm or the nucleus .
	manualset3
217524	8	420142	7	NULL	NULL	0	NULL	free binding sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , U1A represents a novel class of protein which shuttles between cytoplasm and nucleus and whose intracellular distribution can be altered by the number of free binding sites for the protein present in the cytoplasm or the nucleus .
	manualset3
217525	9	420142	7	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , U1A represents a novel class of protein which shuttles between cytoplasm and nucleus and whose intracellular distribution can be altered by the number of free binding sites for the protein present in the cytoplasm or the nucleus .
	manualset3
217526	10	420142	7	NULL	NULL	0	NULL	cytoplasm	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , U1A represents a novel class of protein which shuttles between cytoplasm and nucleus and whose intracellular distribution can be altered by the number of free binding sites for the protein present in the cytoplasm or the nucleus .
	manualset3
217527	11	420142	7	NULL	NULL	0	NULL	nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , U1A represents a novel class of protein which shuttles between cytoplasm and nucleus and whose intracellular distribution can be altered by the number of free binding sites for the protein present in the cytoplasm or the nucleus .
	manualset3
217528	1	420143	7	NULL	NULL	0	NULL	Partial amino acid sequence analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial amino acid sequence analysis of the purified enzyme was conducted and used to plan polymerase chain reaction techniques to clone the MDH3 gene .
	manualset3
217529	2	420143	7	NULL	NULL	0	NULL	 purified enzyme	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial amino acid sequence analysis of the purified enzyme was conducted and used to plan polymerase chain reaction techniques to clone the MDH3 gene .
	manualset3
217530	3	420143	7	NULL	NULL	0	NULL	polymerase chain reaction techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial amino acid sequence analysis of the purified enzyme was conducted and used to plan polymerase chain reaction techniques to clone the MDH3 gene .
	manualset3
217531	4	420143	7	NULL	NULL	0	NULL	MDH3 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Partial amino acid sequence analysis of the purified enzyme was conducted and used to plan polymerase chain reaction techniques to clone the MDH3 gene .
	manualset3
217532	1	420144	7	NULL	NULL	0	NULL	decline 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While there was a decline in basal secretion of inhibin with increasing duration of culture , the capacity of the purified Sertoli cells ( bands 2 and 3 ) to respond to both FSH and dibutyryl cAMP increased over the culture period .
	manualset3
217533	2	420144	7	NULL	NULL	0	NULL	basal secretion 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While there was a decline in basal secretion of inhibin with increasing duration of culture , the capacity of the purified Sertoli cells ( bands 2 and 3 ) to respond to both FSH and dibutyryl cAMP increased over the culture period .
	manualset3
217534	3	420144	7	NULL	NULL	0	NULL	inhibin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	While there was a decline in basal secretion of inhibin with increasing duration of culture , the capacity of the purified Sertoli cells ( bands 2 and 3 ) to respond to both FSH and dibutyryl cAMP increased over the culture period .
	manualset3
217535	4	420144	7	NULL	NULL	0	NULL	increasing duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	While there was a decline in basal secretion of inhibin with increasing duration of culture , the capacity of the purified Sertoli cells ( bands 2 and 3 ) to respond to both FSH and dibutyryl cAMP increased over the culture period .
	manualset3
217536	5	420144	7	NULL	NULL	0	NULL	culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	While there was a decline in basal secretion of inhibin with increasing duration of culture , the capacity of the purified Sertoli cells ( bands 2 and 3 ) to respond to both FSH and dibutyryl cAMP increased over the culture period .
	manualset3
217537	6	420144	7	NULL	NULL	0	NULL	capacity 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	While there was a decline in basal secretion of inhibin with increasing duration of culture , the capacity of the purified Sertoli cells ( bands 2 and 3 ) to respond to both FSH and dibutyryl cAMP increased over the culture period .
	manualset3
217538	7	420144	7	NULL	NULL	0	NULL	purified Sertoli cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	While there was a decline in basal secretion of inhibin with increasing duration of culture , the capacity of the purified Sertoli cells ( bands 2 and 3 ) to respond to both FSH and dibutyryl cAMP increased over the culture period .
	manualset3
217539	8	420144	7	NULL	NULL	0	NULL	bands 2	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	While there was a decline in basal secretion of inhibin with increasing duration of culture , the capacity of the purified Sertoli cells ( bands 2 and 3 ) to respond to both FSH and dibutyryl cAMP increased over the culture period .
	manualset3
217540	9	420144	7	NULL	NULL	0	NULL	bands 3	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	While there was a decline in basal secretion of inhibin with increasing duration of culture , the capacity of the purified Sertoli cells ( bands 2 and 3 ) to respond to both FSH and dibutyryl cAMP increased over the culture period .
	manualset3
217541	10	420144	7	NULL	NULL	0	NULL	FSH 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	While there was a decline in basal secretion of inhibin with increasing duration of culture , the capacity of the purified Sertoli cells ( bands 2 and 3 ) to respond to both FSH and dibutyryl cAMP increased over the culture period .
	manualset3
217542	11	420144	7	NULL	NULL	0	NULL	dibutyryl cAMP 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	While there was a decline in basal secretion of inhibin with increasing duration of culture , the capacity of the purified Sertoli cells ( bands 2 and 3 ) to respond to both FSH and dibutyryl cAMP increased over the culture period .
	manualset3
217543	12	420144	7	NULL	NULL	0	NULL	culture period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	While there was a decline in basal secretion of inhibin with increasing duration of culture , the capacity of the purified Sertoli cells ( bands 2 and 3 ) to respond to both FSH and dibutyryl cAMP increased over the culture period .
	manualset3
217544	1	420145	7	NULL	NULL	0	NULL	standard transabdominal approach 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the standard transabdominal approach is preferred , a variety of approaches , including transgastric , transrectal , transvaginal , and transgluteal , may be used .
	manualset3
217545	2	420145	7	NULL	NULL	0	NULL	approaches	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the standard transabdominal approach is preferred , a variety of approaches , including transgastric , transrectal , transvaginal , and transgluteal , may be used .
	manualset3
217546	3	420145	7	NULL	NULL	0	NULL	transgastric approach	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the standard transabdominal approach is preferred , a variety of approaches , including transgastric , transrectal , transvaginal , and transgluteal , may be used .
	manualset3
217547	4	420145	7	NULL	NULL	0	NULL	transrectal approach	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the standard transabdominal approach is preferred , a variety of approaches , including transgastric , transrectal , transvaginal , and transgluteal , may be used .
	manualset3
217548	5	420145	7	NULL	NULL	0	NULL	transvaginal approach	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the standard transabdominal approach is preferred , a variety of approaches , including transgastric , transrectal , transvaginal , and transgluteal , may be used .
	manualset3
217549	6	420145	7	NULL	NULL	0	NULL	transgluteal approach	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the standard transabdominal approach is preferred , a variety of approaches , including transgastric , transrectal , transvaginal , and transgluteal , may be used .
	manualset3
217559	1	420146	7	NULL	NULL	0	NULL	Bronchial thermoplasty	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Bronchial thermoplasty : a novel treatment for severe asthma requiring monitored anesthesia care .
	manualset3
217560	2	420146	7	NULL	NULL	0	NULL	novel treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Bronchial thermoplasty : a novel treatment for severe asthma requiring monitored anesthesia care .
	manualset3
217561	3	420146	7	NULL	NULL	0	NULL	severe asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Bronchial thermoplasty : a novel treatment for severe asthma requiring monitored anesthesia care .
	manualset3
217562	4	420146	7	NULL	NULL	0	NULL	anesthesia care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Bronchial thermoplasty : a novel treatment for severe asthma requiring monitored anesthesia care .
	manualset3
217563	1	420147	7	NULL	NULL	0	NULL	attitudinal changes	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Favorable attitudinal changes were observed in terms of ` psychiatric services ' , ` human rights of the mentally ill ' , ` patients ' independence in social life ' , and 'cause and characteristics of mental illness ' .
	manualset3
217564	2	420147	7	NULL	NULL	0	NULL	` psychiatric services 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Favorable attitudinal changes were observed in terms of ` psychiatric services ' , ` human rights of the mentally ill ' , ` patients ' independence in social life ' , and 'cause and characteristics of mental illness ' .
	manualset3
217565	3	420147	7	NULL	NULL	0	NULL	 human rights	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Favorable attitudinal changes were observed in terms of ` psychiatric services ' , ` human rights of the mentally ill ' , ` patients ' independence in social life ' , and 'cause and characteristics of mental illness ' .
	manualset3
217566	4	420147	7	NULL	NULL	0	NULL	mentally ill	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Favorable attitudinal changes were observed in terms of ` psychiatric services ' , ` human rights of the mentally ill ' , ` patients ' independence in social life ' , and 'cause and characteristics of mental illness ' .
	manualset3
217567	5	420147	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Favorable attitudinal changes were observed in terms of ` psychiatric services ' , ` human rights of the mentally ill ' , ` patients ' independence in social life ' , and 'cause and characteristics of mental illness ' .
	manualset3
217568	6	420147	7	NULL	NULL	0	NULL	social life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Favorable attitudinal changes were observed in terms of ` psychiatric services ' , ` human rights of the mentally ill ' , ` patients ' independence in social life ' , and 'cause and characteristics of mental illness ' .
	manualset3
217569	7	420147	7	NULL	NULL	0	NULL	cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Favorable attitudinal changes were observed in terms of ` psychiatric services ' , ` human rights of the mentally ill ' , ` patients ' independence in social life ' , and 'cause and characteristics of mental illness ' .
	manualset3
217570	8	420147	7	NULL	NULL	0	NULL	characteristics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Favorable attitudinal changes were observed in terms of ` psychiatric services ' , ` human rights of the mentally ill ' , ` patients ' independence in social life ' , and 'cause and characteristics of mental illness ' .
	manualset3
217571	9	420147	7	NULL	NULL	0	NULL	mental illness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Favorable attitudinal changes were observed in terms of ` psychiatric services ' , ` human rights of the mentally ill ' , ` patients ' independence in social life ' , and 'cause and characteristics of mental illness ' .
	manualset3
217572	1	420148	7	NULL	NULL	0	NULL	Fibrous osteitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Fibrous osteitis was demonstrated in three patients .
	manualset3
217573	2	420148	7	NULL	NULL	0	NULL	three patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Fibrous osteitis was demonstrated in three patients .
	manualset3
217578	1	420149	7	NULL	NULL	0	NULL	first application 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This is the first application of the sensitivity encoding algorithm to characterize the structure of the water resonance at high spatial resolution .
	manualset3
217580	2	420149	7	NULL	NULL	0	NULL	sensitivity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This is the first application of the sensitivity encoding algorithm to characterize the structure of the water resonance at high spatial resolution .
	manualset3
217581	3	420149	7	NULL	NULL	0	NULL	algorithm	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This is the first application of the sensitivity encoding algorithm to characterize the structure of the water resonance at high spatial resolution .
	manualset3
217583	4	420149	7	NULL	NULL	0	NULL	structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	This is the first application of the sensitivity encoding algorithm to characterize the structure of the water resonance at high spatial resolution .
	manualset3
217584	5	420149	7	NULL	NULL	0	NULL	 water resonance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This is the first application of the sensitivity encoding algorithm to characterize the structure of the water resonance at high spatial resolution .
	manualset3
217585	6	420149	7	NULL	NULL	0	NULL	high spatial resolution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This is the first application of the sensitivity encoding algorithm to characterize the structure of the water resonance at high spatial resolution .
	manualset3
217586	1	420150	7	NULL	NULL	0	NULL	Detection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Detection and characterization of a novel branching enzyme from hen oviduct , UDP-N-acetylglucosamine : GlcNAc beta 1-6 ( GlcNAc beta 1-2 ) Man alpha-R ( GlcNAc to Man ) beta-4-N-acetylglucosaminyltransferase VI .
	manualset3
217588	2	420150	7	NULL	NULL	0	NULL	characterization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Detection and characterization of a novel branching enzyme from hen oviduct , UDP-N-acetylglucosamine : GlcNAc beta 1-6 ( GlcNAc beta 1-2 ) Man alpha-R ( GlcNAc to Man ) beta-4-N-acetylglucosaminyltransferase VI .
	manualset3
217590	3	420150	7	NULL	NULL	0	NULL	novel branching enzyme	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Detection and characterization of a novel branching enzyme from hen oviduct , UDP-N-acetylglucosamine : GlcNAc beta 1-6 ( GlcNAc beta 1-2 ) Man alpha-R ( GlcNAc to Man ) beta-4-N-acetylglucosaminyltransferase VI .
	manualset3
217591	4	420150	7	NULL	NULL	0	NULL	hen oviduct	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Detection and characterization of a novel branching enzyme from hen oviduct , UDP-N-acetylglucosamine : GlcNAc beta 1-6 ( GlcNAc beta 1-2 ) Man alpha-R ( GlcNAc to Man ) beta-4-N-acetylglucosaminyltransferase VI .
	manualset3
217625	5	420150	7	NULL	NULL	0	NULL	UDP-N-acetylglucosamine	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Detection and characterization of a novel branching enzyme from hen oviduct , UDP-N-acetylglucosamine : GlcNAc beta 1-6 ( GlcNAc beta 1-2 ) Man alpha-R ( GlcNAc to Man ) beta-4-N-acetylglucosaminyltransferase VI .
	manualset3
217626	6	420150	7	NULL	NULL	0	NULL	GlcNAc beta 1-6 ( GlcNAc beta 1-2 ) Man alpha-R ( GlcNAc to Man ) beta-4-N-acetylglucosaminyltransferase VI	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Detection and characterization of a novel branching enzyme from hen oviduct , UDP-N-acetylglucosamine : GlcNAc beta 1-6 ( GlcNAc beta 1-2 ) Man alpha-R ( GlcNAc to Man ) beta-4-N-acetylglucosaminyltransferase VI .
	manualset3
217627	1	420151	7	NULL	NULL	0	NULL	testosterone response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the testosterone response to human chorionic gonadotropin was normal in all three patients , none of them responded to the antiestrogen , clomiphene .
	manualset3
217628	2	420151	7	NULL	NULL	0	NULL	human chorionic gonadotropin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the testosterone response to human chorionic gonadotropin was normal in all three patients , none of them responded to the antiestrogen , clomiphene .
	manualset3
217629	3	420151	7	NULL	NULL	0	NULL	 three patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the testosterone response to human chorionic gonadotropin was normal in all three patients , none of them responded to the antiestrogen , clomiphene .
	manualset3
217630	4	420151	7	NULL	NULL	0	NULL	antiestrogen	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the testosterone response to human chorionic gonadotropin was normal in all three patients , none of them responded to the antiestrogen , clomiphene .
	manualset3
217631	5	420151	7	NULL	NULL	0	NULL	clomiphene	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the testosterone response to human chorionic gonadotropin was normal in all three patients , none of them responded to the antiestrogen , clomiphene .
	manualset3
217649	1	420152	7	NULL	NULL	0	NULL	Cardiac Cycle	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Cardiac Cycle is a Major Contributor to Variability in Size Measurements of Abdominal Aortic Aneurysms by Ultrasound .
	manualset3
217650	2	420152	7	NULL	NULL	0	NULL	Major Contributor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Cardiac Cycle is a Major Contributor to Variability in Size Measurements of Abdominal Aortic Aneurysms by Ultrasound .
	manualset3
217651	3	420152	7	NULL	NULL	0	NULL	Variability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Cardiac Cycle is a Major Contributor to Variability in Size Measurements of Abdominal Aortic Aneurysms by Ultrasound .
	manualset3
217652	4	420152	7	NULL	NULL	0	NULL	Size Measurements	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Cardiac Cycle is a Major Contributor to Variability in Size Measurements of Abdominal Aortic Aneurysms by Ultrasound .
	manualset3
217653	5	420152	7	NULL	NULL	0	NULL	Abdominal Aortic Aneurysms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Cardiac Cycle is a Major Contributor to Variability in Size Measurements of Abdominal Aortic Aneurysms by Ultrasound .
	manualset3
217654	6	420152	7	NULL	NULL	0	NULL	Ultrasound	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The Cardiac Cycle is a Major Contributor to Variability in Size Measurements of Abdominal Aortic Aneurysms by Ultrasound .
	manualset3
217655	1	420153	7	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors evaluate the relation of ethnic , socioeconomic status ( SES ) , and belief match between parents and group leaders and engagement in a preventive intervention for parents of preschoolers .
	manualset3
217656	2	420153	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors evaluate the relation of ethnic , socioeconomic status ( SES ) , and belief match between parents and group leaders and engagement in a preventive intervention for parents of preschoolers .
	manualset3
217657	3	420153	7	NULL	NULL	NULL	NULL	ethnic status	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The authors evaluate the relation of ethnic , socioeconomic status ( SES ) , and belief match between parents and group leaders and engagement in a preventive intervention for parents of preschoolers .
	manualset3
217658	4	420153	7	NULL	NULL	0	NULL	socioeconomic status ( SES )	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors evaluate the relation of ethnic , socioeconomic status ( SES ) , and belief match between parents and group leaders and engagement in a preventive intervention for parents of preschoolers .
	manualset3
217659	5	420153	7	NULL	NULL	0	NULL	belief match	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors evaluate the relation of ethnic , socioeconomic status ( SES ) , and belief match between parents and group leaders and engagement in a preventive intervention for parents of preschoolers .
	manualset3
217660	6	420153	7	NULL	NULL	0	NULL	parents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors evaluate the relation of ethnic , socioeconomic status ( SES ) , and belief match between parents and group leaders and engagement in a preventive intervention for parents of preschoolers .
	manualset3
217661	7	420153	7	NULL	NULL	0	NULL	group leaders	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors evaluate the relation of ethnic , socioeconomic status ( SES ) , and belief match between parents and group leaders and engagement in a preventive intervention for parents of preschoolers .
	manualset3
217662	8	420153	7	NULL	NULL	0	NULL	engagement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors evaluate the relation of ethnic , socioeconomic status ( SES ) , and belief match between parents and group leaders and engagement in a preventive intervention for parents of preschoolers .
	manualset3
217663	9	420153	7	NULL	NULL	0	NULL	preventive intervention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors evaluate the relation of ethnic , socioeconomic status ( SES ) , and belief match between parents and group leaders and engagement in a preventive intervention for parents of preschoolers .
	manualset3
217664	10	420153	7	NULL	NULL	0	NULL	parents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors evaluate the relation of ethnic , socioeconomic status ( SES ) , and belief match between parents and group leaders and engagement in a preventive intervention for parents of preschoolers .
	manualset3
217665	11	420153	7	NULL	NULL	0	NULL	preschoolers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors evaluate the relation of ethnic , socioeconomic status ( SES ) , and belief match between parents and group leaders and engagement in a preventive intervention for parents of preschoolers .
	manualset3
217666	1	420154	7	NULL	NULL	0	NULL	Tomography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Tomography of the canaliculus vestibuli ) .
	manualset3
217667	2	420154	7	NULL	NULL	0	NULL	canaliculus vestibuli 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Tomography of the canaliculus vestibuli ) .
	manualset3
217668	1	420155	7	NULL	NULL	0	NULL	Clonus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Clonus was apparently suppressed by electrical stimulation in an area ( F , 10.0 mm ; L , 4.0 mm ; D , from +2 to -2 ; there was especially marked suppression of clonus by stimulation in sub-VL .
	manualset3
217669	2	420155	7	NULL	NULL	0	NULL	electrical stimulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Clonus was apparently suppressed by electrical stimulation in an area ( F , 10.0 mm ; L , 4.0 mm ; D , from +2 to -2 ; there was especially marked suppression of clonus by stimulation in sub-VL .
	manualset3
217670	3	420155	7	NULL	NULL	0	NULL	area 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Clonus was apparently suppressed by electrical stimulation in an area ( F , 10.0 mm ; L , 4.0 mm ; D , from +2 to -2 ; there was especially marked suppression of clonus by stimulation in sub-VL .
	manualset3
217671	4	420155	7	NULL	NULL	0	NULL	F , 10.0 mm 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Clonus was apparently suppressed by electrical stimulation in an area ( F , 10.0 mm ; L , 4.0 mm ; D , from +2 to -2 ; there was especially marked suppression of clonus by stimulation in sub-VL .
	manualset3
217672	5	420155	7	NULL	NULL	0	NULL	L , 4.0 mm	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Clonus was apparently suppressed by electrical stimulation in an area ( F , 10.0 mm ; L , 4.0 mm ; D , from +2 to -2 ; there was especially marked suppression of clonus by stimulation in sub-VL .
	manualset3
217673	6	420155	7	NULL	NULL	0	NULL	D , from +2 to -2 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Clonus was apparently suppressed by electrical stimulation in an area ( F , 10.0 mm ; L , 4.0 mm ; D , from +2 to -2 ; there was especially marked suppression of clonus by stimulation in sub-VL .
	manualset3
217674	7	420155	7	NULL	NULL	0	NULL	suppression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Clonus was apparently suppressed by electrical stimulation in an area ( F , 10.0 mm ; L , 4.0 mm ; D , from +2 to -2 ; there was especially marked suppression of clonus by stimulation in sub-VL .
	manualset3
217675	8	420155	7	NULL	NULL	0	NULL	clonus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Clonus was apparently suppressed by electrical stimulation in an area ( F , 10.0 mm ; L , 4.0 mm ; D , from +2 to -2 ; there was especially marked suppression of clonus by stimulation in sub-VL .
	manualset3
217676	9	420155	7	NULL	NULL	0	NULL	stimulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Clonus was apparently suppressed by electrical stimulation in an area ( F , 10.0 mm ; L , 4.0 mm ; D , from +2 to -2 ; there was especially marked suppression of clonus by stimulation in sub-VL .
	manualset3
217677	10	420155	7	NULL	NULL	0	NULL	sub-VL 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Clonus was apparently suppressed by electrical stimulation in an area ( F , 10.0 mm ; L , 4.0 mm ; D , from +2 to -2 ; there was especially marked suppression of clonus by stimulation in sub-VL .
	manualset3
217678	1	420156	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the autoimmune disorder on pregnancy and the effects of pregnancy on the course of the autoimmune disorder are also discussed with an emphasis on the implications for clinical management .
	manualset3
217679	2	420156	7	NULL	NULL	0	NULL	autoimmune disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the autoimmune disorder on pregnancy and the effects of pregnancy on the course of the autoimmune disorder are also discussed with an emphasis on the implications for clinical management .
	manualset3
217680	3	420156	7	NULL	NULL	0	NULL	 pregnancy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the autoimmune disorder on pregnancy and the effects of pregnancy on the course of the autoimmune disorder are also discussed with an emphasis on the implications for clinical management .
	manualset3
217681	4	420156	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the autoimmune disorder on pregnancy and the effects of pregnancy on the course of the autoimmune disorder are also discussed with an emphasis on the implications for clinical management .
	manualset3
217682	5	420156	7	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the autoimmune disorder on pregnancy and the effects of pregnancy on the course of the autoimmune disorder are also discussed with an emphasis on the implications for clinical management .
	manualset3
217683	6	420156	7	NULL	NULL	0	NULL	course	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the autoimmune disorder on pregnancy and the effects of pregnancy on the course of the autoimmune disorder are also discussed with an emphasis on the implications for clinical management .
	manualset3
217684	7	420156	7	NULL	NULL	0	NULL	autoimmune disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the autoimmune disorder on pregnancy and the effects of pregnancy on the course of the autoimmune disorder are also discussed with an emphasis on the implications for clinical management .
	manualset3
217685	8	420156	7	NULL	NULL	0	NULL	emphasis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the autoimmune disorder on pregnancy and the effects of pregnancy on the course of the autoimmune disorder are also discussed with an emphasis on the implications for clinical management .
	manualset3
217686	9	420156	7	NULL	NULL	0	NULL	 implications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the autoimmune disorder on pregnancy and the effects of pregnancy on the course of the autoimmune disorder are also discussed with an emphasis on the implications for clinical management .
	manualset3
217687	10	420156	7	NULL	NULL	0	NULL	clinical management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the autoimmune disorder on pregnancy and the effects of pregnancy on the course of the autoimmune disorder are also discussed with an emphasis on the implications for clinical management .
	manualset3
217688	1	420157	7	NULL	NULL	0	NULL	unilateral spatial neglect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the unilateral spatial neglect was improving , the patient was unable to paint the left quarter of a watercolor , but there was no error in line drawing .
	manualset3
217689	2	420157	7	NULL	NULL	0	NULL	 patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the unilateral spatial neglect was improving , the patient was unable to paint the left quarter of a watercolor , but there was no error in line drawing .
	manualset3
217690	3	420157	7	NULL	NULL	0	NULL	left quarter 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the unilateral spatial neglect was improving , the patient was unable to paint the left quarter of a watercolor , but there was no error in line drawing .
	manualset3
217691	4	420157	7	NULL	NULL	0	NULL	 watercolor	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the unilateral spatial neglect was improving , the patient was unable to paint the left quarter of a watercolor , but there was no error in line drawing .
	manualset3
217692	5	420157	7	NULL	NULL	0	NULL	no error	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the unilateral spatial neglect was improving , the patient was unable to paint the left quarter of a watercolor , but there was no error in line drawing .
	manualset3
217693	6	420157	7	NULL	NULL	0	NULL	line drawing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the unilateral spatial neglect was improving , the patient was unable to paint the left quarter of a watercolor , but there was no error in line drawing .
	manualset3
217694	1	420158	7	NULL	NULL	0	NULL	mean follow-up	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	At a mean follow-up of nine years ( 2 to 12 ) , two patients had been lost to follow-up , and three await a second-stage procedure .
	manualset3
217695	2	420158	7	NULL	NULL	0	NULL	 nine years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	At a mean follow-up of nine years ( 2 to 12 ) , two patients had been lost to follow-up , and three await a second-stage procedure .
	manualset3
217696	3	420158	7	NULL	NULL	0	NULL	 2 to 12	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	At a mean follow-up of nine years ( 2 to 12 ) , two patients had been lost to follow-up , and three await a second-stage procedure .
	manualset3
217697	4	420158	7	NULL	NULL	0	NULL	 two patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	At a mean follow-up of nine years ( 2 to 12 ) , two patients had been lost to follow-up , and three await a second-stage procedure .
	manualset3
217698	5	420158	7	NULL	NULL	0	NULL	follow-up	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	At a mean follow-up of nine years ( 2 to 12 ) , two patients had been lost to follow-up , and three await a second-stage procedure .
	manualset3
217699	6	420158	7	NULL	NULL	0	NULL	three 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	At a mean follow-up of nine years ( 2 to 12 ) , two patients had been lost to follow-up , and three await a second-stage procedure .
	manualset3
217700	7	420158	7	NULL	NULL	0	NULL	second-stage procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	At a mean follow-up of nine years ( 2 to 12 ) , two patients had been lost to follow-up , and three await a second-stage procedure .
	manualset3
217701	1	420159	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings present the first evidence that phages infecting GB-124 are inactivated by the levels of UV-C radiation routinely delivered during tertiary wastewater treatment processes .
	manualset3
217702	2	420159	7	NULL	NULL	0	NULL	first evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings present the first evidence that phages infecting GB-124 are inactivated by the levels of UV-C radiation routinely delivered during tertiary wastewater treatment processes .
	manualset3
217703	3	420159	7	NULL	NULL	0	NULL	phages 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings present the first evidence that phages infecting GB-124 are inactivated by the levels of UV-C radiation routinely delivered during tertiary wastewater treatment processes .
	manualset3
217704	4	420159	7	NULL	NULL	0	NULL	GB-124	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings present the first evidence that phages infecting GB-124 are inactivated by the levels of UV-C radiation routinely delivered during tertiary wastewater treatment processes .
	manualset3
217705	5	420159	7	NULL	NULL	0	NULL	 levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings present the first evidence that phages infecting GB-124 are inactivated by the levels of UV-C radiation routinely delivered during tertiary wastewater treatment processes .
	manualset3
217706	6	420159	7	NULL	NULL	0	NULL	UV-C radiation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings present the first evidence that phages infecting GB-124 are inactivated by the levels of UV-C radiation routinely delivered during tertiary wastewater treatment processes .
	manualset3
217707	7	420159	7	NULL	NULL	0	NULL	 tertiary wastewater treatment processes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These findings present the first evidence that phages infecting GB-124 are inactivated by the levels of UV-C radiation routinely delivered during tertiary wastewater treatment processes .
	manualset3
217708	1	420160	7	NULL	NULL	0	NULL	de-epithelialized transverse rectus abdominis musculocutaneous flap	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A de-epithelialized transverse rectus abdominis musculocutaneous flap is then used to fill the empty `` skin brassiere , '' effectively replacing the glandular defect , and a small patch of skin is exteriorized to match the areolar defect .
	manualset3
217709	2	420160	7	NULL	NULL	0	NULL	`` skin brassiere "	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A de-epithelialized transverse rectus abdominis musculocutaneous flap is then used to fill the empty `` skin brassiere , '' effectively replacing the glandular defect , and a small patch of skin is exteriorized to match the areolar defect .
	manualset3
217710	3	420160	7	NULL	NULL	0	NULL	glandular defect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A de-epithelialized transverse rectus abdominis musculocutaneous flap is then used to fill the empty `` skin brassiere , '' effectively replacing the glandular defect , and a small patch of skin is exteriorized to match the areolar defect .
	manualset3
217711	4	420160	7	NULL	NULL	0	NULL	small patch of skin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A de-epithelialized transverse rectus abdominis musculocutaneous flap is then used to fill the empty `` skin brassiere , '' effectively replacing the glandular defect , and a small patch of skin is exteriorized to match the areolar defect .
	manualset3
217712	5	420160	7	NULL	NULL	0	NULL	areolar defect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A de-epithelialized transverse rectus abdominis musculocutaneous flap is then used to fill the empty `` skin brassiere , '' effectively replacing the glandular defect , and a small patch of skin is exteriorized to match the areolar defect .
	manualset3
217713	1	420161	7	NULL	NULL	0	NULL	Teeth 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Teeth and toothache in the history of dentistry ) .
	manualset3
217714	2	420161	7	NULL	NULL	0	NULL	toothache	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Teeth and toothache in the history of dentistry ) .
	manualset3
217715	3	420161	7	NULL	NULL	0	NULL	history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Teeth and toothache in the history of dentistry ) .
	manualset3
217716	4	420161	7	NULL	NULL	0	NULL	dentistry	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Teeth and toothache in the history of dentistry ) .
	manualset3
217717	1	420162	7	NULL	NULL	0	NULL	in vitro finding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This in vitro finding is promising for potential use of topical tea tree oil formulations in the treatment of candidiasis due to fluconazole-resistant strains .
	manualset3
217718	2	420162	7	NULL	NULL	0	NULL	potential use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This in vitro finding is promising for potential use of topical tea tree oil formulations in the treatment of candidiasis due to fluconazole-resistant strains .
	manualset3
217719	3	420162	7	NULL	NULL	0	NULL	topical tea tree oil formulations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This in vitro finding is promising for potential use of topical tea tree oil formulations in the treatment of candidiasis due to fluconazole-resistant strains .
	manualset3
217720	4	420162	7	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This in vitro finding is promising for potential use of topical tea tree oil formulations in the treatment of candidiasis due to fluconazole-resistant strains .
	manualset3
217721	5	420162	7	NULL	NULL	0	NULL	candidiasis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This in vitro finding is promising for potential use of topical tea tree oil formulations in the treatment of candidiasis due to fluconazole-resistant strains .
	manualset3
217722	6	420162	7	NULL	NULL	0	NULL	fluconazole-resistant strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	This in vitro finding is promising for potential use of topical tea tree oil formulations in the treatment of candidiasis due to fluconazole-resistant strains .
	manualset3
217723	1	420163	7	NULL	NULL	0	NULL	Causes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Causes of poor performance of horses during training , racing , or showing : 348 cases ( 1992-1996 ) .
	manualset3
217724	2	420163	7	NULL	NULL	0	NULL	poor performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Causes of poor performance of horses during training , racing , or showing : 348 cases ( 1992-1996 ) .
	manualset3
217725	3	420163	7	NULL	NULL	0	NULL	horses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Causes of poor performance of horses during training , racing , or showing : 348 cases ( 1992-1996 ) .
	manualset3
217726	4	420163	7	NULL	NULL	0	NULL	training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Causes of poor performance of horses during training , racing , or showing : 348 cases ( 1992-1996 ) .
	manualset3
217727	5	420163	7	NULL	NULL	0	NULL	racing 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Causes of poor performance of horses during training , racing , or showing : 348 cases ( 1992-1996 ) .
	manualset3
217728	6	420163	7	NULL	NULL	0	NULL	showing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Causes of poor performance of horses during training , racing , or showing : 348 cases ( 1992-1996 ) .
	manualset3
217729	7	420163	7	NULL	NULL	NULL	NULL	348 cases	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Causes of poor performance of horses during training , racing , or showing : 348 cases ( 1992-1996 ) .
	manualset3
217730	8	420163	7	NULL	NULL	0	NULL	1992-1996	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Causes of poor performance of horses during training , racing , or showing : 348 cases ( 1992-1996 ) .
	manualset3
217731	1	420164	7	NULL	NULL	0	NULL	 trends	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These trends reflect population aging , smoking patterns , institutional factors , and treatment practices .
	manualset3
217732	2	420164	7	NULL	NULL	0	NULL	 population aging	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These trends reflect population aging , smoking patterns , institutional factors , and treatment practices .
	manualset3
217733	3	420164	7	NULL	NULL	0	NULL	 smoking patterns	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These trends reflect population aging , smoking patterns , institutional factors , and treatment practices .
	manualset3
217734	4	420164	7	NULL	NULL	0	NULL	institutional factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These trends reflect population aging , smoking patterns , institutional factors , and treatment practices .
	manualset3
217735	5	420164	7	NULL	NULL	0	NULL	treatment practices	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	These trends reflect population aging , smoking patterns , institutional factors , and treatment practices .
	manualset3
217736	1	420165	7	NULL	NULL	NULL	NULL	Adverse reactions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Adverse reactions required interruption of treatment in 64 patients on goldsalts ( 35.2 % ) , in 44 on levamisole ( 31.7 % ) and in 5 on D-Penicillamine ( 20.8 % ) .
	manualset3
217737	2	420165	7	NULL	NULL	0	NULL	interruption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Adverse reactions required interruption of treatment in 64 patients on goldsalts ( 35.2 % ) , in 44 on levamisole ( 31.7 % ) and in 5 on D-Penicillamine ( 20.8 % ) .
	manualset3
217738	3	420165	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Adverse reactions required interruption of treatment in 64 patients on goldsalts ( 35.2 % ) , in 44 on levamisole ( 31.7 % ) and in 5 on D-Penicillamine ( 20.8 % ) .
	manualset3
217739	4	420165	7	NULL	NULL	0	NULL	64 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Adverse reactions required interruption of treatment in 64 patients on goldsalts ( 35.2 % ) , in 44 on levamisole ( 31.7 % ) and in 5 on D-Penicillamine ( 20.8 % ) .
	manualset3
217740	5	420165	7	NULL	NULL	0	NULL	goldsalts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Adverse reactions required interruption of treatment in 64 patients on goldsalts ( 35.2 % ) , in 44 on levamisole ( 31.7 % ) and in 5 on D-Penicillamine ( 20.8 % ) .
	manualset3
217741	6	420165	7	NULL	NULL	0	NULL	35.2 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Adverse reactions required interruption of treatment in 64 patients on goldsalts ( 35.2 % ) , in 44 on levamisole ( 31.7 % ) and in 5 on D-Penicillamine ( 20.8 % ) .
	manualset3
217742	7	420165	7	NULL	NULL	0	NULL	44 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Adverse reactions required interruption of treatment in 64 patients on goldsalts ( 35.2 % ) , in 44 on levamisole ( 31.7 % ) and in 5 on D-Penicillamine ( 20.8 % ) .
	manualset3
217743	8	420165	7	NULL	NULL	0	NULL	levamisole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Adverse reactions required interruption of treatment in 64 patients on goldsalts ( 35.2 % ) , in 44 on levamisole ( 31.7 % ) and in 5 on D-Penicillamine ( 20.8 % ) .
	manualset3
217744	9	420165	7	NULL	NULL	0	NULL	31.7 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Adverse reactions required interruption of treatment in 64 patients on goldsalts ( 35.2 % ) , in 44 on levamisole ( 31.7 % ) and in 5 on D-Penicillamine ( 20.8 % ) .
	manualset3
217745	10	420165	7	NULL	NULL	0	NULL	 5 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Adverse reactions required interruption of treatment in 64 patients on goldsalts ( 35.2 % ) , in 44 on levamisole ( 31.7 % ) and in 5 on D-Penicillamine ( 20.8 % ) .
	manualset3
217746	11	420165	7	NULL	NULL	0	NULL	D-Penicillamine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Adverse reactions required interruption of treatment in 64 patients on goldsalts ( 35.2 % ) , in 44 on levamisole ( 31.7 % ) and in 5 on D-Penicillamine ( 20.8 % ) .
	manualset3
217747	12	420165	7	NULL	NULL	0	NULL	20.8 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Adverse reactions required interruption of treatment in 64 patients on goldsalts ( 35.2 % ) , in 44 on levamisole ( 31.7 % ) and in 5 on D-Penicillamine ( 20.8 % ) .
	manualset3
217748	1	420166	7	NULL	NULL	0	NULL	fasting levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The fasting and incremental postprandial levels of insulin , C-peptide , glucagon , and somatostatin did not change , whereas the mean triglyceride concentrations were lower after the high-fiber diet .
	manualset3
217749	2	420166	7	NULL	NULL	0	NULL	 incremental postprandial levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The fasting and incremental postprandial levels of insulin , C-peptide , glucagon , and somatostatin did not change , whereas the mean triglyceride concentrations were lower after the high-fiber diet .
	manualset3
217750	3	420166	7	NULL	NULL	0	NULL	insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The fasting and incremental postprandial levels of insulin , C-peptide , glucagon , and somatostatin did not change , whereas the mean triglyceride concentrations were lower after the high-fiber diet .
	manualset3
217751	4	420166	7	NULL	NULL	0	NULL	C-peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The fasting and incremental postprandial levels of insulin , C-peptide , glucagon , and somatostatin did not change , whereas the mean triglyceride concentrations were lower after the high-fiber diet .
	manualset3
217752	5	420166	7	NULL	NULL	0	NULL	glucagon	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The fasting and incremental postprandial levels of insulin , C-peptide , glucagon , and somatostatin did not change , whereas the mean triglyceride concentrations were lower after the high-fiber diet .
	manualset3
217753	6	420166	7	NULL	NULL	0	NULL	somatostatin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The fasting and incremental postprandial levels of insulin , C-peptide , glucagon , and somatostatin did not change , whereas the mean triglyceride concentrations were lower after the high-fiber diet .
	manualset3
217754	7	420166	7	NULL	NULL	0	NULL	mean triglyceride concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The fasting and incremental postprandial levels of insulin , C-peptide , glucagon , and somatostatin did not change , whereas the mean triglyceride concentrations were lower after the high-fiber diet .
	manualset3
217755	8	420166	7	NULL	NULL	0	NULL	high-fiber diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The fasting and incremental postprandial levels of insulin , C-peptide , glucagon , and somatostatin did not change , whereas the mean triglyceride concentrations were lower after the high-fiber diet .
	manualset3
217756	1	420167	7	NULL	NULL	0	NULL	KLIMOVAN INJECTION	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( KLIMOVAN INJECTION AS A DIAGNOSTIC METHOD IN PREGNANCY ) .
	manualset3
217757	2	420167	7	NULL	NULL	NULL	NULL	DIAGNOSTIC METHOD	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( KLIMOVAN INJECTION AS A DIAGNOSTIC METHOD IN PREGNANCY ) .
	manualset3
217758	3	420167	7	NULL	NULL	0	NULL	PREGNANCY	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( KLIMOVAN INJECTION AS A DIAGNOSTIC METHOD IN PREGNANCY ) .
	manualset3
217759	1	420168	7	NULL	NULL	0	NULL	carbon dioxide laser surgical unit 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The carbon dioxide laser surgical unit as an instrument for surgery of brain tumors -- its advantages and disadvantages .
	manualset3
217760	2	420168	7	NULL	NULL	0	NULL	 instrument 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The carbon dioxide laser surgical unit as an instrument for surgery of brain tumors -- its advantages and disadvantages .
	manualset3
217761	3	420168	7	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The carbon dioxide laser surgical unit as an instrument for surgery of brain tumors -- its advantages and disadvantages .
	manualset3
217762	4	420168	7	NULL	NULL	0	NULL	brain tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The carbon dioxide laser surgical unit as an instrument for surgery of brain tumors -- its advantages and disadvantages .
	manualset3
217763	1	420169	7	NULL	NULL	0	NULL	3-day limitation	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	This 3-day limitation is based on the biochemical and physiological changes that occur during storage and that result in decreased viability and survival after transfusion .
	manualset3
217764	2	420169	7	NULL	NULL	0	NULL	biochemical changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This 3-day limitation is based on the biochemical and physiological changes that occur during storage and that result in decreased viability and survival after transfusion .
	manualset3
217765	3	420169	7	NULL	NULL	0	NULL	physiological changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This 3-day limitation is based on the biochemical and physiological changes that occur during storage and that result in decreased viability and survival after transfusion .
	manualset3
217766	4	420169	7	NULL	NULL	0	NULL	storage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This 3-day limitation is based on the biochemical and physiological changes that occur during storage and that result in decreased viability and survival after transfusion .
	manualset3
217767	5	420169	7	NULL	NULL	0	NULL	decreased viability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This 3-day limitation is based on the biochemical and physiological changes that occur during storage and that result in decreased viability and survival after transfusion .
	manualset3
217768	6	420169	7	NULL	NULL	0	NULL	survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This 3-day limitation is based on the biochemical and physiological changes that occur during storage and that result in decreased viability and survival after transfusion .
	manualset3
217769	7	420169	7	NULL	NULL	0	NULL	transfusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This 3-day limitation is based on the biochemical and physiological changes that occur during storage and that result in decreased viability and survival after transfusion .
	manualset3
217770	1	420170	7	NULL	NULL	0	NULL	Experimentally induced susceptibility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Experimentally induced susceptibility to audiogenic seizure .
	manualset3
217771	2	420170	7	NULL	NULL	0	NULL	audiogenic seizure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Experimentally induced susceptibility to audiogenic seizure .
	manualset3
217772	1	420171	7	NULL	NULL	0	NULL	37 degrees C	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	At 37 degrees C , cell-bound EGF : ferritin rapidly redistributed in the plane of the plasma membrane to form small groups that were subsequently internalized into pinocytic vesicles .
	manualset3
217773	2	420171	7	NULL	NULL	0	NULL	cell-bound EGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	At 37 degrees C , cell-bound EGF : ferritin rapidly redistributed in the plane of the plasma membrane to form small groups that were subsequently internalized into pinocytic vesicles .
	manualset3
217774	3	420171	7	NULL	NULL	0	NULL	ferritin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	At 37 degrees C , cell-bound EGF : ferritin rapidly redistributed in the plane of the plasma membrane to form small groups that were subsequently internalized into pinocytic vesicles .
	manualset3
217775	4	420171	7	NULL	NULL	0	NULL	plane of the plasma membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	At 37 degrees C , cell-bound EGF : ferritin rapidly redistributed in the plane of the plasma membrane to form small groups that were subsequently internalized into pinocytic vesicles .
	manualset3
217776	5	420171	7	NULL	NULL	0	NULL	small groups	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	At 37 degrees C , cell-bound EGF : ferritin rapidly redistributed in the plane of the plasma membrane to form small groups that were subsequently internalized into pinocytic vesicles .
	manualset3
217777	6	420171	7	NULL	NULL	0	NULL	pinocytic vesicles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	At 37 degrees C , cell-bound EGF : ferritin rapidly redistributed in the plane of the plasma membrane to form small groups that were subsequently internalized into pinocytic vesicles .
	manualset3
217778	1	420172	7	NULL	NULL	0	NULL	highly conserved enhancer	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A highly conserved enhancer in the Dlx5/Dlx6 intergenic region is the site of cross-regulatory interactions between Dlx genes in the embryonic forebrain .
	manualset3
217779	2	420172	7	NULL	NULL	0	NULL	Dlx5/Dlx6 intergenic region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A highly conserved enhancer in the Dlx5/Dlx6 intergenic region is the site of cross-regulatory interactions between Dlx genes in the embryonic forebrain .
	manualset3
217780	3	420172	7	NULL	NULL	0	NULL	 site	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A highly conserved enhancer in the Dlx5/Dlx6 intergenic region is the site of cross-regulatory interactions between Dlx genes in the embryonic forebrain .
	manualset3
217781	4	420172	7	NULL	NULL	0	NULL	cross-regulatory interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A highly conserved enhancer in the Dlx5/Dlx6 intergenic region is the site of cross-regulatory interactions between Dlx genes in the embryonic forebrain .
	manualset3
217782	5	420172	7	NULL	NULL	0	NULL	Dlx genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A highly conserved enhancer in the Dlx5/Dlx6 intergenic region is the site of cross-regulatory interactions between Dlx genes in the embryonic forebrain .
	manualset3
217783	6	420172	7	NULL	NULL	0	NULL	embryonic forebrain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A highly conserved enhancer in the Dlx5/Dlx6 intergenic region is the site of cross-regulatory interactions between Dlx genes in the embryonic forebrain .
	manualset3
217784	1	420173	7	NULL	NULL	0	NULL	commonly-used method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A commonly-used method for testing for association between disease and a single-nucleotide polymorphism ( SNP ) is to compare the frequencies of the SNP genotypes in a sample of unrelated cases to those in a sample of unrelated controls drawn from the same population ( an unmatched case-control study ) .
	manualset3
217785	2	420173	7	NULL	NULL	0	NULL	testing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A commonly-used method for testing for association between disease and a single-nucleotide polymorphism ( SNP ) is to compare the frequencies of the SNP genotypes in a sample of unrelated cases to those in a sample of unrelated controls drawn from the same population ( an unmatched case-control study ) .
	manualset3
217786	3	420173	7	NULL	NULL	0	NULL	association	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A commonly-used method for testing for association between disease and a single-nucleotide polymorphism ( SNP ) is to compare the frequencies of the SNP genotypes in a sample of unrelated cases to those in a sample of unrelated controls drawn from the same population ( an unmatched case-control study ) .
	manualset3
217787	4	420173	7	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A commonly-used method for testing for association between disease and a single-nucleotide polymorphism ( SNP ) is to compare the frequencies of the SNP genotypes in a sample of unrelated cases to those in a sample of unrelated controls drawn from the same population ( an unmatched case-control study ) .
	manualset3
217788	5	420173	7	NULL	NULL	0	NULL	single-nucleotide polymorphism ( SNP )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A commonly-used method for testing for association between disease and a single-nucleotide polymorphism ( SNP ) is to compare the frequencies of the SNP genotypes in a sample of unrelated cases to those in a sample of unrelated controls drawn from the same population ( an unmatched case-control study ) .
	manualset3
217789	6	420173	7	NULL	NULL	0	NULL	frequencies	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A commonly-used method for testing for association between disease and a single-nucleotide polymorphism ( SNP ) is to compare the frequencies of the SNP genotypes in a sample of unrelated cases to those in a sample of unrelated controls drawn from the same population ( an unmatched case-control study ) .
	manualset3
217790	7	420173	7	NULL	NULL	0	NULL	SNP genotypes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A commonly-used method for testing for association between disease and a single-nucleotide polymorphism ( SNP ) is to compare the frequencies of the SNP genotypes in a sample of unrelated cases to those in a sample of unrelated controls drawn from the same population ( an unmatched case-control study ) .
	manualset3
217791	8	420173	7	NULL	NULL	0	NULL	sample	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A commonly-used method for testing for association between disease and a single-nucleotide polymorphism ( SNP ) is to compare the frequencies of the SNP genotypes in a sample of unrelated cases to those in a sample of unrelated controls drawn from the same population ( an unmatched case-control study ) .
	manualset3
217792	9	420173	7	NULL	NULL	0	NULL	unrelated cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A commonly-used method for testing for association between disease and a single-nucleotide polymorphism ( SNP ) is to compare the frequencies of the SNP genotypes in a sample of unrelated cases to those in a sample of unrelated controls drawn from the same population ( an unmatched case-control study ) .
	manualset3
217793	10	420173	7	NULL	NULL	0	NULL	 sample	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A commonly-used method for testing for association between disease and a single-nucleotide polymorphism ( SNP ) is to compare the frequencies of the SNP genotypes in a sample of unrelated cases to those in a sample of unrelated controls drawn from the same population ( an unmatched case-control study ) .
	manualset3
217794	11	420173	7	NULL	NULL	0	NULL	unrelated controls	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A commonly-used method for testing for association between disease and a single-nucleotide polymorphism ( SNP ) is to compare the frequencies of the SNP genotypes in a sample of unrelated cases to those in a sample of unrelated controls drawn from the same population ( an unmatched case-control study ) .
	manualset3
217795	12	420173	7	NULL	NULL	0	NULL	same population 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A commonly-used method for testing for association between disease and a single-nucleotide polymorphism ( SNP ) is to compare the frequencies of the SNP genotypes in a sample of unrelated cases to those in a sample of unrelated controls drawn from the same population ( an unmatched case-control study ) .
	manualset3
217796	13	420173	7	NULL	NULL	0	NULL	unmatched case-control study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A commonly-used method for testing for association between disease and a single-nucleotide polymorphism ( SNP ) is to compare the frequencies of the SNP genotypes in a sample of unrelated cases to those in a sample of unrelated controls drawn from the same population ( an unmatched case-control study ) .
	manualset3
217797	1	420174	7	NULL	NULL	NULL	NULL	Emerson effect	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The Emerson effect was observed as an enhancement of photosynthesis in long wavelength red light ( 700 mmicro ) when shorter wavelengths were added .
	manualset3
217798	2	420174	7	NULL	NULL	0	NULL	enhancement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Emerson effect was observed as an enhancement of photosynthesis in long wavelength red light ( 700 mmicro ) when shorter wavelengths were added .
	manualset3
217799	3	420174	7	NULL	NULL	0	NULL	photosynthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Emerson effect was observed as an enhancement of photosynthesis in long wavelength red light ( 700 mmicro ) when shorter wavelengths were added .
	manualset3
217800	4	420174	7	NULL	NULL	0	NULL	long wavelength red light	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The Emerson effect was observed as an enhancement of photosynthesis in long wavelength red light ( 700 mmicro ) when shorter wavelengths were added .
	manualset3
217801	5	420174	7	NULL	NULL	0	NULL	700 mmicro	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Emerson effect was observed as an enhancement of photosynthesis in long wavelength red light ( 700 mmicro ) when shorter wavelengths were added .
	manualset3
217802	6	420174	7	NULL	NULL	0	NULL	shorter wavelengths	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Emerson effect was observed as an enhancement of photosynthesis in long wavelength red light ( 700 mmicro ) when shorter wavelengths were added .
	manualset3
217803	1	420175	7	NULL	NULL	0	NULL	questions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there are some questions concerning the relationship of antibody levels to protection , the low antibody responses in this study are an indication that R75 is not sufficiently immunogenic .
	manualset3
217804	2	420175	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there are some questions concerning the relationship of antibody levels to protection , the low antibody responses in this study are an indication that R75 is not sufficiently immunogenic .
	manualset3
217805	3	420175	7	NULL	NULL	0	NULL	antibody levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there are some questions concerning the relationship of antibody levels to protection , the low antibody responses in this study are an indication that R75 is not sufficiently immunogenic .
	manualset3
217806	4	420175	7	NULL	NULL	0	NULL	 protection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there are some questions concerning the relationship of antibody levels to protection , the low antibody responses in this study are an indication that R75 is not sufficiently immunogenic .
	manualset3
217807	5	420175	7	NULL	NULL	0	NULL	low antibody responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there are some questions concerning the relationship of antibody levels to protection , the low antibody responses in this study are an indication that R75 is not sufficiently immunogenic .
	manualset3
217808	6	420175	7	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there are some questions concerning the relationship of antibody levels to protection , the low antibody responses in this study are an indication that R75 is not sufficiently immunogenic .
	manualset3
217809	7	420175	7	NULL	NULL	0	NULL	indication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there are some questions concerning the relationship of antibody levels to protection , the low antibody responses in this study are an indication that R75 is not sufficiently immunogenic .
	manualset3
217810	8	420175	7	NULL	NULL	0	NULL	R75	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there are some questions concerning the relationship of antibody levels to protection , the low antibody responses in this study are an indication that R75 is not sufficiently immunogenic .
	manualset3
217811	9	420175	7	NULL	NULL	0	NULL	immunogenic 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there are some questions concerning the relationship of antibody levels to protection , the low antibody responses in this study are an indication that R75 is not sufficiently immunogenic .
	manualset3
217812	1	420176	7	NULL	NULL	0	NULL	Expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of retinoic acid receptor genes in neural crest-derived cells during mouse facial development .
	manualset3
217813	2	420176	7	NULL	NULL	0	NULL	retinoic acid receptor genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of retinoic acid receptor genes in neural crest-derived cells during mouse facial development .
	manualset3
217814	3	420176	7	NULL	NULL	0	NULL	neural crest-derived cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of retinoic acid receptor genes in neural crest-derived cells during mouse facial development .
	manualset3
217815	4	420176	7	NULL	NULL	0	NULL	mouse facial development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of retinoic acid receptor genes in neural crest-derived cells during mouse facial development .
	manualset3
217816	1	420177	7	NULL	NULL	NULL	NULL	Stage IV-S neuroblastoma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Stage IV-S neuroblastoma , characterized by a primary tumor plus disseminated tumors in liver , skin and bone marrow , has a favorable clinical prognosis when compared to metastatic Stage IV neuroblastoma .
	manualset3
217817	2	420177	7	NULL	NULL	0	NULL	primary tumor plus disseminated tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Stage IV-S neuroblastoma , characterized by a primary tumor plus disseminated tumors in liver , skin and bone marrow , has a favorable clinical prognosis when compared to metastatic Stage IV neuroblastoma .
	manualset3
217818	3	420177	7	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Stage IV-S neuroblastoma , characterized by a primary tumor plus disseminated tumors in liver , skin and bone marrow , has a favorable clinical prognosis when compared to metastatic Stage IV neuroblastoma .
	manualset3
217819	4	420177	7	NULL	NULL	0	NULL	skin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Stage IV-S neuroblastoma , characterized by a primary tumor plus disseminated tumors in liver , skin and bone marrow , has a favorable clinical prognosis when compared to metastatic Stage IV neuroblastoma .
	manualset3
217820	5	420177	7	NULL	NULL	0	NULL	bone marrow	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Stage IV-S neuroblastoma , characterized by a primary tumor plus disseminated tumors in liver , skin and bone marrow , has a favorable clinical prognosis when compared to metastatic Stage IV neuroblastoma .
	manualset3
217821	6	420177	7	NULL	NULL	0	NULL	clinical prognosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Stage IV-S neuroblastoma , characterized by a primary tumor plus disseminated tumors in liver , skin and bone marrow , has a favorable clinical prognosis when compared to metastatic Stage IV neuroblastoma .
	manualset3
217822	7	420177	7	NULL	NULL	0	NULL	metastatic Stage IV neuroblastoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Stage IV-S neuroblastoma , characterized by a primary tumor plus disseminated tumors in liver , skin and bone marrow , has a favorable clinical prognosis when compared to metastatic Stage IV neuroblastoma .
	manualset3
217823	1	420178	7	NULL	NULL	0	NULL	historical HIT cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with historical HIT cases , the rate of thrombosis was reduced from 50 % to 29 % ( p = 0.39 ) during surveillance .
	manualset3
217824	2	420178	7	NULL	NULL	0	NULL	rate 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with historical HIT cases , the rate of thrombosis was reduced from 50 % to 29 % ( p = 0.39 ) during surveillance .
	manualset3
217825	3	420178	7	NULL	NULL	0	NULL	thrombosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with historical HIT cases , the rate of thrombosis was reduced from 50 % to 29 % ( p = 0.39 ) during surveillance .
	manualset3
217826	4	420178	7	NULL	NULL	0	NULL	50 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with historical HIT cases , the rate of thrombosis was reduced from 50 % to 29 % ( p = 0.39 ) during surveillance .
	manualset3
217827	5	420178	7	NULL	NULL	0	NULL	29 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with historical HIT cases , the rate of thrombosis was reduced from 50 % to 29 % ( p = 0.39 ) during surveillance .
	manualset3
217828	6	420178	7	NULL	NULL	0	NULL	 p = 0.39	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with historical HIT cases , the rate of thrombosis was reduced from 50 % to 29 % ( p = 0.39 ) during surveillance .
	manualset3
217829	7	420178	7	NULL	NULL	0	NULL	surveillance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with historical HIT cases , the rate of thrombosis was reduced from 50 % to 29 % ( p = 0.39 ) during surveillance .
	manualset3
217830	1	420179	7	NULL	NULL	0	NULL	Biphasic peroxidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Biphasic peroxidase in the study of Fc receptors of leukemic lymphocytes ) .
	manualset3
217831	2	420179	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Biphasic peroxidase in the study of Fc receptors of leukemic lymphocytes ) .
	manualset3
217832	3	420179	7	NULL	NULL	0	NULL	Fc receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Biphasic peroxidase in the study of Fc receptors of leukemic lymphocytes ) .
	manualset3
217833	4	420179	7	NULL	NULL	0	NULL	leukemic lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	( Biphasic peroxidase in the study of Fc receptors of leukemic lymphocytes ) .
	manualset3
217867	1	420180	7	NULL	NULL	0	NULL	Determination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Determination of dimethyl sulfoxide and dimethyl sulfone in urine by gas chromatography-mass spectrometry after preparation using 2 , 2-dimethoxypropane .
	manualset3
217868	2	420180	7	NULL	NULL	0	NULL	dimethyl sulfoxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Determination of dimethyl sulfoxide and dimethyl sulfone in urine by gas chromatography-mass spectrometry after preparation using 2 , 2-dimethoxypropane .
	manualset3
217869	3	420180	7	NULL	NULL	0	NULL	dimethyl sulfone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Determination of dimethyl sulfoxide and dimethyl sulfone in urine by gas chromatography-mass spectrometry after preparation using 2 , 2-dimethoxypropane .
	manualset3
217870	4	420180	7	NULL	NULL	0	NULL	urine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Determination of dimethyl sulfoxide and dimethyl sulfone in urine by gas chromatography-mass spectrometry after preparation using 2 , 2-dimethoxypropane .
	manualset3
217871	5	420180	7	NULL	NULL	0	NULL	gas chromatography-mass spectrometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Determination of dimethyl sulfoxide and dimethyl sulfone in urine by gas chromatography-mass spectrometry after preparation using 2 , 2-dimethoxypropane .
	manualset3
217872	6	420180	7	NULL	NULL	0	NULL	preparation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Determination of dimethyl sulfoxide and dimethyl sulfone in urine by gas chromatography-mass spectrometry after preparation using 2 , 2-dimethoxypropane .
	manualset3
217873	7	420180	7	NULL	NULL	0	NULL	2 , 2-dimethoxypropane	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Determination of dimethyl sulfoxide and dimethyl sulfone in urine by gas chromatography-mass spectrometry after preparation using 2 , 2-dimethoxypropane .
	manualset3
217874	1	420181	7	NULL	NULL	0	NULL	 potential use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential use of the PBIS as a research and clinical instrument is discussed .
	manualset3
217875	2	420181	7	NULL	NULL	0	NULL	 PBIS 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential use of the PBIS as a research and clinical instrument is discussed .
	manualset3
217876	3	420181	7	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential use of the PBIS as a research and clinical instrument is discussed .
	manualset3
217877	4	420181	7	NULL	NULL	0	NULL	clinical instrument 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The potential use of the PBIS as a research and clinical instrument is discussed .
	manualset3
217878	1	420182	7	NULL	NULL	0	NULL	incidents	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there clearly have been incidents of abuse in these relationships , academic-industrial collaboration is an engine that drives innovation in the biomedical sciences in this country .
	manualset3
217879	2	420182	7	NULL	NULL	0	NULL	abuse	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there clearly have been incidents of abuse in these relationships , academic-industrial collaboration is an engine that drives innovation in the biomedical sciences in this country .
	manualset3
217880	3	420182	7	NULL	NULL	NULL	NULL	relationships	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although there clearly have been incidents of abuse in these relationships , academic-industrial collaboration is an engine that drives innovation in the biomedical sciences in this country .
	manualset3
217881	4	420182	7	NULL	NULL	0	NULL	academic-industrial collaboration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there clearly have been incidents of abuse in these relationships , academic-industrial collaboration is an engine that drives innovation in the biomedical sciences in this country .
	manualset3
217882	5	420182	7	NULL	NULL	0	NULL	engine	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there clearly have been incidents of abuse in these relationships , academic-industrial collaboration is an engine that drives innovation in the biomedical sciences in this country .
	manualset3
217883	6	420182	7	NULL	NULL	0	NULL	 innovation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there clearly have been incidents of abuse in these relationships , academic-industrial collaboration is an engine that drives innovation in the biomedical sciences in this country .
	manualset3
217884	7	420182	7	NULL	NULL	0	NULL	biomedical sciences	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there clearly have been incidents of abuse in these relationships , academic-industrial collaboration is an engine that drives innovation in the biomedical sciences in this country .
	manualset3
217885	8	420182	7	NULL	NULL	0	NULL	country 	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there clearly have been incidents of abuse in these relationships , academic-industrial collaboration is an engine that drives innovation in the biomedical sciences in this country .
	manualset3
217886	1	420183	7	NULL	NULL	0	NULL	rare instance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We describe a rare instance of a patient who developed an RVOT aneurysm after trans-ventricular repair of tetralogy of Fallot , which was complicated with the formation of a thrombus in the aneurysm sac .
	manualset3
217887	2	420183	7	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	We describe a rare instance of a patient who developed an RVOT aneurysm after trans-ventricular repair of tetralogy of Fallot , which was complicated with the formation of a thrombus in the aneurysm sac .
	manualset3
217888	3	420183	7	NULL	NULL	0	NULL	RVOT aneurysm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We describe a rare instance of a patient who developed an RVOT aneurysm after trans-ventricular repair of tetralogy of Fallot , which was complicated with the formation of a thrombus in the aneurysm sac .
	manualset3
217889	4	420183	7	NULL	NULL	0	NULL	 trans-ventricular repair	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	We describe a rare instance of a patient who developed an RVOT aneurysm after trans-ventricular repair of tetralogy of Fallot , which was complicated with the formation of a thrombus in the aneurysm sac .
	manualset3
217890	5	420183	7	NULL	NULL	0	NULL	tetralogy of Fallot 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We describe a rare instance of a patient who developed an RVOT aneurysm after trans-ventricular repair of tetralogy of Fallot , which was complicated with the formation of a thrombus in the aneurysm sac .
	manualset3
217891	6	420183	7	NULL	NULL	0	NULL	formation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We describe a rare instance of a patient who developed an RVOT aneurysm after trans-ventricular repair of tetralogy of Fallot , which was complicated with the formation of a thrombus in the aneurysm sac .
	manualset3
217892	7	420183	7	NULL	NULL	0	NULL	thrombus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We describe a rare instance of a patient who developed an RVOT aneurysm after trans-ventricular repair of tetralogy of Fallot , which was complicated with the formation of a thrombus in the aneurysm sac .
	manualset3
217893	8	420183	7	NULL	NULL	0	NULL	aneurysm sac	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We describe a rare instance of a patient who developed an RVOT aneurysm after trans-ventricular repair of tetralogy of Fallot , which was complicated with the formation of a thrombus in the aneurysm sac .
	manualset3
217894	1	420184	7	NULL	NULL	0	NULL	alcohol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Avoid or severely restrict alcohol , including wine and beer .
	manualset3
217895	2	420184	7	NULL	NULL	0	NULL	wine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Avoid or severely restrict alcohol , including wine and beer .
	manualset3
217896	3	420184	7	NULL	NULL	0	NULL	 beer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Avoid or severely restrict alcohol , including wine and beer .
	manualset3
217897	1	420185	7	NULL	NULL	0	NULL	strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The strains with the most extensive PCB degradation capacity did strongly hybridize to the bph probe , but a few strains that exhibited strong hybridization had poor PCB-degrading ability .
	manualset3
217898	2	420185	7	NULL	NULL	0	NULL	PCB degradation capacity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The strains with the most extensive PCB degradation capacity did strongly hybridize to the bph probe , but a few strains that exhibited strong hybridization had poor PCB-degrading ability .
	manualset3
217899	3	420185	7	NULL	NULL	0	NULL	bph probe	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The strains with the most extensive PCB degradation capacity did strongly hybridize to the bph probe , but a few strains that exhibited strong hybridization had poor PCB-degrading ability .
	manualset3
217900	4	420185	7	NULL	NULL	0	NULL	few strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The strains with the most extensive PCB degradation capacity did strongly hybridize to the bph probe , but a few strains that exhibited strong hybridization had poor PCB-degrading ability .
	manualset3
217901	5	420185	7	NULL	NULL	0	NULL	strong hybridization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The strains with the most extensive PCB degradation capacity did strongly hybridize to the bph probe , but a few strains that exhibited strong hybridization had poor PCB-degrading ability .
	manualset3
217902	6	420185	7	NULL	NULL	0	NULL	poor PCB-degrading ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The strains with the most extensive PCB degradation capacity did strongly hybridize to the bph probe , but a few strains that exhibited strong hybridization had poor PCB-degrading ability .
	manualset3
217903	1	420186	7	NULL	NULL	0	NULL	Chicken meat	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Chicken meat and eggs contaminated with Salmonella result in economic losses in the poultry industry and potential human infection .
	manualset3
217904	2	420186	7	NULL	NULL	0	NULL	eggs	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Chicken meat and eggs contaminated with Salmonella result in economic losses in the poultry industry and potential human infection .
	manualset3
217905	3	420186	7	NULL	NULL	0	NULL	Salmonella	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Chicken meat and eggs contaminated with Salmonella result in economic losses in the poultry industry and potential human infection .
	manualset3
217906	4	420186	7	NULL	NULL	0	NULL	 poultry industry 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Chicken meat and eggs contaminated with Salmonella result in economic losses in the poultry industry and potential human infection .
	manualset3
217907	5	420186	7	NULL	NULL	0	NULL	 human infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Chicken meat and eggs contaminated with Salmonella result in economic losses in the poultry industry and potential human infection .
	manualset3
217908	6	420186	7	NULL	NULL	0	NULL	economic losses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Chicken meat and eggs contaminated with Salmonella result in economic losses in the poultry industry and potential human infection .
	manualset3
217909	1	420187	7	NULL	NULL	0	NULL	Increased blood pressure recovery	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased blood pressure recovery after stress was also linked to trait forgiveness .
	manualset3
217910	2	420187	7	NULL	NULL	0	NULL	stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased blood pressure recovery after stress was also linked to trait forgiveness .
	manualset3
217911	3	420187	7	NULL	NULL	0	NULL	 trait forgiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased blood pressure recovery after stress was also linked to trait forgiveness .
	manualset3
217912	1	420188	7	NULL	NULL	0	NULL	circular dichroism ( CD )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrate circular dichroism ( CD ) in the second harmonic generation ( SHG ) signal from chiral assemblies of G-shaped nanostructures made of gold .
	manualset3
217913	2	420188	7	NULL	NULL	NULL	NULL	second harmonic generation ( SHG ) signal	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We demonstrate circular dichroism ( CD ) in the second harmonic generation ( SHG ) signal from chiral assemblies of G-shaped nanostructures made of gold .
	manualset3
217914	3	420188	7	NULL	NULL	0	NULL	chiral assemblies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrate circular dichroism ( CD ) in the second harmonic generation ( SHG ) signal from chiral assemblies of G-shaped nanostructures made of gold .
	manualset3
217915	4	420188	7	NULL	NULL	0	NULL	G-shaped nanostructures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrate circular dichroism ( CD ) in the second harmonic generation ( SHG ) signal from chiral assemblies of G-shaped nanostructures made of gold .
	manualset3
217916	5	420188	7	NULL	NULL	0	NULL	gold 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrate circular dichroism ( CD ) in the second harmonic generation ( SHG ) signal from chiral assemblies of G-shaped nanostructures made of gold .
	manualset3
217918	1	420189	7	NULL	NULL	0	NULL	obtainment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This includes the obtainment of photographs and detailed documentation of the burn injury .
	manualset3
217919	2	420189	7	NULL	NULL	0	NULL	photographs	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	This includes the obtainment of photographs and detailed documentation of the burn injury .
	manualset3
217920	3	420189	7	NULL	NULL	0	NULL	 detailed documentation	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This includes the obtainment of photographs and detailed documentation of the burn injury .
	manualset3
217921	4	420189	7	NULL	NULL	0	NULL	burn injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This includes the obtainment of photographs and detailed documentation of the burn injury .
	manualset3
217922	1	420190	7	NULL	NULL	0	NULL	Accumulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Accumulation of guanosine tetraphosphate during leucine starvation showed no correlation with the amount of DNA synthesized .
	manualset3
217923	2	420190	7	NULL	NULL	0	NULL	guanosine tetraphosphate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Accumulation of guanosine tetraphosphate during leucine starvation showed no correlation with the amount of DNA synthesized .
	manualset3
217924	3	420190	7	NULL	NULL	0	NULL	leucine starvation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Accumulation of guanosine tetraphosphate during leucine starvation showed no correlation with the amount of DNA synthesized .
	manualset3
217925	4	420190	7	NULL	NULL	0	NULL	no correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Accumulation of guanosine tetraphosphate during leucine starvation showed no correlation with the amount of DNA synthesized .
	manualset3
217926	5	420190	7	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Accumulation of guanosine tetraphosphate during leucine starvation showed no correlation with the amount of DNA synthesized .
	manualset3
217927	6	420190	7	NULL	NULL	NULL	NULL	DNA	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Accumulation of guanosine tetraphosphate during leucine starvation showed no correlation with the amount of DNA synthesized .
	manualset3
217928	1	420191	7	NULL	NULL	0	NULL	Feline leukemia virus-free lymphosarcoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Feline leukemia virus-free lymphosarcoma in a specific pathogen free cat .
	manualset3
217929	2	420191	7	NULL	NULL	0	NULL	specific pathogen free cat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Feline leukemia virus-free lymphosarcoma in a specific pathogen free cat .
	manualset3
217931	1	420192	7	NULL	NULL	0	NULL	NEW METABOLIC DISEASE	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( A NEW METABOLIC DISEASE OF ERYTHROCYTIC MANIFESTATION : ERYTHROPOIETIC PROTOPORPHYRIA ) .
	manualset3
217932	2	420192	7	NULL	NULL	0	NULL	ERYTHROCYTIC MANIFESTATION	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( A NEW METABOLIC DISEASE OF ERYTHROCYTIC MANIFESTATION : ERYTHROPOIETIC PROTOPORPHYRIA ) .
	manualset3
217933	3	420192	7	NULL	NULL	0	NULL	ERYTHROPOIETIC PROTOPORPHYRIA	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( A NEW METABOLIC DISEASE OF ERYTHROCYTIC MANIFESTATION : ERYTHROPOIETIC PROTOPORPHYRIA ) .
	manualset3
217934	1	420193	7	NULL	NULL	0	NULL	Data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Data on the detection of glaucoma in polyclinics of Samarkand ) .
	manualset3
217935	2	420193	7	NULL	NULL	0	NULL	detection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Data on the detection of glaucoma in polyclinics of Samarkand ) .
	manualset3
217936	3	420193	7	NULL	NULL	0	NULL	glaucoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Data on the detection of glaucoma in polyclinics of Samarkand ) .
	manualset3
217937	4	420193	7	NULL	NULL	0	NULL	polyclinics	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( Data on the detection of glaucoma in polyclinics of Samarkand ) .
	manualset3
217938	5	420193	7	NULL	NULL	0	NULL	Samarkand 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Data on the detection of glaucoma in polyclinics of Samarkand ) .
	manualset3
217939	1	420194	7	NULL	NULL	0	NULL	Information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Information on reproductive health , occupational exposure history , and other covariates including age at pregnancy , time and duration of leave from job since pregnancy , and mill location was obtained by trained nurses with a standardised questionnaire .
	manualset3
217940	2	420194	7	NULL	NULL	0	NULL	reproductive health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Information on reproductive health , occupational exposure history , and other covariates including age at pregnancy , time and duration of leave from job since pregnancy , and mill location was obtained by trained nurses with a standardised questionnaire .
	manualset3
217941	3	420194	7	NULL	NULL	0	NULL	occupational exposure history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Information on reproductive health , occupational exposure history , and other covariates including age at pregnancy , time and duration of leave from job since pregnancy , and mill location was obtained by trained nurses with a standardised questionnaire .
	manualset3
217942	4	420194	7	NULL	NULL	0	NULL	covariates	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Information on reproductive health , occupational exposure history , and other covariates including age at pregnancy , time and duration of leave from job since pregnancy , and mill location was obtained by trained nurses with a standardised questionnaire .
	manualset3
217943	5	420194	7	NULL	NULL	0	NULL	age	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Information on reproductive health , occupational exposure history , and other covariates including age at pregnancy , time and duration of leave from job since pregnancy , and mill location was obtained by trained nurses with a standardised questionnaire .
	manualset3
217944	6	420194	7	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Information on reproductive health , occupational exposure history , and other covariates including age at pregnancy , time and duration of leave from job since pregnancy , and mill location was obtained by trained nurses with a standardised questionnaire .
	manualset3
217945	7	420194	7	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Information on reproductive health , occupational exposure history , and other covariates including age at pregnancy , time and duration of leave from job since pregnancy , and mill location was obtained by trained nurses with a standardised questionnaire .
	manualset3
217946	8	420194	7	NULL	NULL	0	NULL	duration 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Information on reproductive health , occupational exposure history , and other covariates including age at pregnancy , time and duration of leave from job since pregnancy , and mill location was obtained by trained nurses with a standardised questionnaire .
	manualset3
217947	9	420194	7	NULL	NULL	0	NULL	 leave	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Information on reproductive health , occupational exposure history , and other covariates including age at pregnancy , time and duration of leave from job since pregnancy , and mill location was obtained by trained nurses with a standardised questionnaire .
	manualset3
217948	10	420194	7	NULL	NULL	0	NULL	job	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Information on reproductive health , occupational exposure history , and other covariates including age at pregnancy , time and duration of leave from job since pregnancy , and mill location was obtained by trained nurses with a standardised questionnaire .
	manualset3
217949	11	420194	7	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Information on reproductive health , occupational exposure history , and other covariates including age at pregnancy , time and duration of leave from job since pregnancy , and mill location was obtained by trained nurses with a standardised questionnaire .
	manualset3
217950	12	420194	7	NULL	NULL	0	NULL	mill location 	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Information on reproductive health , occupational exposure history , and other covariates including age at pregnancy , time and duration of leave from job since pregnancy , and mill location was obtained by trained nurses with a standardised questionnaire .
	manualset3
217951	13	420194	7	NULL	NULL	0	NULL	 trained nurses	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Information on reproductive health , occupational exposure history , and other covariates including age at pregnancy , time and duration of leave from job since pregnancy , and mill location was obtained by trained nurses with a standardised questionnaire .
	manualset3
217952	14	420194	7	NULL	NULL	0	NULL	standardised questionnaire	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Information on reproductive health , occupational exposure history , and other covariates including age at pregnancy , time and duration of leave from job since pregnancy , and mill location was obtained by trained nurses with a standardised questionnaire .
	manualset3
217953	1	420195	7	NULL	NULL	NULL	NULL	new member 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A new member of the HDGF family in humans and mice was identified and cloned ; we call it HRP-3 .
	manualset3
217954	2	420195	7	NULL	NULL	NULL	NULL	HDGF family	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A new member of the HDGF family in humans and mice was identified and cloned ; we call it HRP-3 .
	manualset3
217955	3	420195	7	NULL	NULL	0	NULL	humans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A new member of the HDGF family in humans and mice was identified and cloned ; we call it HRP-3 .
	manualset3
217956	4	420195	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A new member of the HDGF family in humans and mice was identified and cloned ; we call it HRP-3 .
	manualset3
217957	5	420195	7	NULL	NULL	0	NULL	HRP-3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A new member of the HDGF family in humans and mice was identified and cloned ; we call it HRP-3 .
	manualset3
217958	1	420196	7	NULL	NULL	0	NULL	32 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 32 high MSI cancers , 13 cancers ( 40.6 % ) harbored at least one of AXIN2 and TCF7L2 mutation , whereas 19 cancers ( 59.4 % ) harbored neither .
	manualset3
217959	2	420196	7	NULL	NULL	0	NULL	high MSI cancers	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 32 high MSI cancers , 13 cancers ( 40.6 % ) harbored at least one of AXIN2 and TCF7L2 mutation , whereas 19 cancers ( 59.4 % ) harbored neither .
	manualset3
217960	3	420196	7	NULL	NULL	0	NULL	13 cancers 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 32 high MSI cancers , 13 cancers ( 40.6 % ) harbored at least one of AXIN2 and TCF7L2 mutation , whereas 19 cancers ( 59.4 % ) harbored neither .
	manualset3
217961	4	420196	7	NULL	NULL	0	NULL	40.6 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 32 high MSI cancers , 13 cancers ( 40.6 % ) harbored at least one of AXIN2 and TCF7L2 mutation , whereas 19 cancers ( 59.4 % ) harbored neither .
	manualset3
217962	5	420196	7	NULL	NULL	0	NULL	 AXIN2 mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 32 high MSI cancers , 13 cancers ( 40.6 % ) harbored at least one of AXIN2 and TCF7L2 mutation , whereas 19 cancers ( 59.4 % ) harbored neither .
	manualset3
217963	6	420196	7	NULL	NULL	0	NULL	 TCF7L2 mutation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 32 high MSI cancers , 13 cancers ( 40.6 % ) harbored at least one of AXIN2 and TCF7L2 mutation , whereas 19 cancers ( 59.4 % ) harbored neither .
	manualset3
217964	7	420196	7	NULL	NULL	0	NULL	19 cancers 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 32 high MSI cancers , 13 cancers ( 40.6 % ) harbored at least one of AXIN2 and TCF7L2 mutation , whereas 19 cancers ( 59.4 % ) harbored neither .
	manualset3
217965	8	420196	7	NULL	NULL	0	NULL	59.4 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 32 high MSI cancers , 13 cancers ( 40.6 % ) harbored at least one of AXIN2 and TCF7L2 mutation , whereas 19 cancers ( 59.4 % ) harbored neither .
	manualset3
217966	1	420197	7	NULL	NULL	0	NULL	substance	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The substance was injected into the bladder neck region of a series of dogs .
	manualset3
217967	2	420197	7	NULL	NULL	0	NULL	bladder neck region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The substance was injected into the bladder neck region of a series of dogs .
	manualset3
217968	3	420197	7	NULL	NULL	0	NULL	series of dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The substance was injected into the bladder neck region of a series of dogs .
	manualset3
217969	1	420198	7	NULL	NULL	0	NULL	Variations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Variations of the RF with pH during paper chromatography of pterines ) .
	manualset3
217970	2	420198	7	NULL	NULL	0	NULL	 RF	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Variations of the RF with pH during paper chromatography of pterines ) .
	manualset3
217971	3	420198	7	NULL	NULL	0	NULL	pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Variations of the RF with pH during paper chromatography of pterines ) .
	manualset3
217972	4	420198	7	NULL	NULL	0	NULL	paper chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Variations of the RF with pH during paper chromatography of pterines ) .
	manualset3
217973	5	420198	7	NULL	NULL	0	NULL	pterines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Variations of the RF with pH during paper chromatography of pterines ) .
	manualset3
217974	1	420199	7	NULL	NULL	0	NULL	image analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using image analysis to quantify the morphological change , we have demonstrated that the effect of AC toxin on cell spreading is dose dependent .
	manualset3
217975	2	420199	7	NULL	NULL	0	NULL	morphological change 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using image analysis to quantify the morphological change , we have demonstrated that the effect of AC toxin on cell spreading is dose dependent .
	manualset3
217976	3	420199	7	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using image analysis to quantify the morphological change , we have demonstrated that the effect of AC toxin on cell spreading is dose dependent .
	manualset3
217977	4	420199	7	NULL	NULL	0	NULL	AC toxin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using image analysis to quantify the morphological change , we have demonstrated that the effect of AC toxin on cell spreading is dose dependent .
	manualset3
217978	5	420199	7	NULL	NULL	0	NULL	cell spreading	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using image analysis to quantify the morphological change , we have demonstrated that the effect of AC toxin on cell spreading is dose dependent .
	manualset3
217979	6	420199	7	NULL	NULL	0	NULL	dose dependent 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using image analysis to quantify the morphological change , we have demonstrated that the effect of AC toxin on cell spreading is dose dependent .
	manualset3
217980	1	420200	7	NULL	NULL	0	NULL	imaging findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The imaging findings of a crack cocaine `` body stuffer '' are presented along with findings from in vitro experimentation with crack cocaine .
	manualset3
217981	2	420200	7	NULL	NULL	0	NULL	crack cocaine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The imaging findings of a crack cocaine `` body stuffer '' are presented along with findings from in vitro experimentation with crack cocaine .
	manualset3
217982	3	420200	7	NULL	NULL	0	NULL	body stuffer	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The imaging findings of a crack cocaine `` body stuffer '' are presented along with findings from in vitro experimentation with crack cocaine .
	manualset3
217983	4	420200	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The imaging findings of a crack cocaine `` body stuffer '' are presented along with findings from in vitro experimentation with crack cocaine .
	manualset3
217984	5	420200	7	NULL	NULL	0	NULL	in vitro experimentation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The imaging findings of a crack cocaine `` body stuffer '' are presented along with findings from in vitro experimentation with crack cocaine .
	manualset3
217985	6	420200	7	NULL	NULL	0	NULL	crack cocaine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The imaging findings of a crack cocaine `` body stuffer '' are presented along with findings from in vitro experimentation with crack cocaine .
	manualset3
217986	1	420201	7	NULL	NULL	0	NULL	agreement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there has been agreement that enteral nutrition remains an excellent means of providing nutritional support to malnourished patients with normal or near normal gastrointestinal function , it is clear that areas of controversy do exist , and attention needs to be directed towards these in the future .
	manualset3
217987	2	420201	7	NULL	NULL	NULL	NULL	enteral nutrition	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although there has been agreement that enteral nutrition remains an excellent means of providing nutritional support to malnourished patients with normal or near normal gastrointestinal function , it is clear that areas of controversy do exist , and attention needs to be directed towards these in the future .
	manualset3
217989	3	420201	7	NULL	NULL	0	NULL	nutritional support	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there has been agreement that enteral nutrition remains an excellent means of providing nutritional support to malnourished patients with normal or near normal gastrointestinal function , it is clear that areas of controversy do exist , and attention needs to be directed towards these in the future .
	manualset3
217990	4	420201	7	NULL	NULL	0	NULL	malnourished patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there has been agreement that enteral nutrition remains an excellent means of providing nutritional support to malnourished patients with normal or near normal gastrointestinal function , it is clear that areas of controversy do exist , and attention needs to be directed towards these in the future .
	manualset3
217991	5	420201	7	NULL	NULL	NULL	NULL	normal gastrointestinal function	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although there has been agreement that enteral nutrition remains an excellent means of providing nutritional support to malnourished patients with normal or near normal gastrointestinal function , it is clear that areas of controversy do exist , and attention needs to be directed towards these in the future .
	manualset3
217992	6	420201	7	NULL	NULL	NULL	NULL	areas of controversy	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although there has been agreement that enteral nutrition remains an excellent means of providing nutritional support to malnourished patients with normal or near normal gastrointestinal function , it is clear that areas of controversy do exist , and attention needs to be directed towards these in the future .
	manualset3
217993	7	420201	7	NULL	NULL	0	NULL	attention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there has been agreement that enteral nutrition remains an excellent means of providing nutritional support to malnourished patients with normal or near normal gastrointestinal function , it is clear that areas of controversy do exist , and attention needs to be directed towards these in the future .
	manualset3
217994	8	420201	7	NULL	NULL	NULL	NULL	future	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although there has been agreement that enteral nutrition remains an excellent means of providing nutritional support to malnourished patients with normal or near normal gastrointestinal function , it is clear that areas of controversy do exist , and attention needs to be directed towards these in the future .
	manualset3
217995	1	420202	7	NULL	NULL	0	NULL	basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of RSM and experimental evidence , the optimum derivatization conditions were defined as reaction temperature of 75C , reaction duration of 70 min , BSTFA reagent concentration of 55 % and pyridine concentration of 35 % .
	manualset3
217996	2	420202	7	NULL	NULL	0	NULL	RSM	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of RSM and experimental evidence , the optimum derivatization conditions were defined as reaction temperature of 75C , reaction duration of 70 min , BSTFA reagent concentration of 55 % and pyridine concentration of 35 % .
	manualset3
217997	3	420202	7	NULL	NULL	0	NULL	 experimental evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of RSM and experimental evidence , the optimum derivatization conditions were defined as reaction temperature of 75C , reaction duration of 70 min , BSTFA reagent concentration of 55 % and pyridine concentration of 35 % .
	manualset3
217998	4	420202	7	NULL	NULL	0	NULL	optimum derivatization conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of RSM and experimental evidence , the optimum derivatization conditions were defined as reaction temperature of 75C , reaction duration of 70 min , BSTFA reagent concentration of 55 % and pyridine concentration of 35 % .
	manualset3
217999	5	420202	7	NULL	NULL	NULL	NULL	reaction temperature	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On the basis of RSM and experimental evidence , the optimum derivatization conditions were defined as reaction temperature of 75C , reaction duration of 70 min , BSTFA reagent concentration of 55 % and pyridine concentration of 35 % .
	manualset3
218000	6	420202	7	NULL	NULL	0	NULL	75C	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of RSM and experimental evidence , the optimum derivatization conditions were defined as reaction temperature of 75C , reaction duration of 70 min , BSTFA reagent concentration of 55 % and pyridine concentration of 35 % .
	manualset3
218001	7	420202	7	NULL	NULL	0	NULL	reaction duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of RSM and experimental evidence , the optimum derivatization conditions were defined as reaction temperature of 75C , reaction duration of 70 min , BSTFA reagent concentration of 55 % and pyridine concentration of 35 % .
	manualset3
218002	8	420202	7	NULL	NULL	0	NULL	70 min 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of RSM and experimental evidence , the optimum derivatization conditions were defined as reaction temperature of 75C , reaction duration of 70 min , BSTFA reagent concentration of 55 % and pyridine concentration of 35 % .
	manualset3
218003	9	420202	7	NULL	NULL	0	NULL	BSTFA reagent concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of RSM and experimental evidence , the optimum derivatization conditions were defined as reaction temperature of 75C , reaction duration of 70 min , BSTFA reagent concentration of 55 % and pyridine concentration of 35 % .
	manualset3
218004	10	420202	7	NULL	NULL	0	NULL	 55 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of RSM and experimental evidence , the optimum derivatization conditions were defined as reaction temperature of 75C , reaction duration of 70 min , BSTFA reagent concentration of 55 % and pyridine concentration of 35 % .
	manualset3
218005	11	420202	7	NULL	NULL	0	NULL	pyridine concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of RSM and experimental evidence , the optimum derivatization conditions were defined as reaction temperature of 75C , reaction duration of 70 min , BSTFA reagent concentration of 55 % and pyridine concentration of 35 % .
	manualset3
218006	12	420202	7	NULL	NULL	0	NULL	35 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of RSM and experimental evidence , the optimum derivatization conditions were defined as reaction temperature of 75C , reaction duration of 70 min , BSTFA reagent concentration of 55 % and pyridine concentration of 35 % .
	manualset3
218007	1	420203	7	NULL	NULL	0	NULL	validity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The validity and usefulness of the end-tidal pCO 2 during anaesthesia .
	manualset3
218008	2	420203	7	NULL	NULL	0	NULL	usefulness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The validity and usefulness of the end-tidal pCO 2 during anaesthesia .
	manualset3
218009	3	420203	7	NULL	NULL	0	NULL	end-tidal pCO 2	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The validity and usefulness of the end-tidal pCO 2 during anaesthesia .
	manualset3
218010	4	420203	7	NULL	NULL	0	NULL	anaesthesia	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The validity and usefulness of the end-tidal pCO 2 during anaesthesia .
	manualset3
218011	1	420204	7	NULL	NULL	NULL	NULL	Serology	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Serology for infectious diseases included blue-tongue , brucellosis , bovine respiratory syncytial virus infection , bovine viral diarrhea/mucosal disease , infectious bovine rhinotracheitis , Johne 's disease ( paratuberculosis ) , foot and mouth disease ( FMD ) , leptospirosis ( eight serovars ) , epizootic hemorrhagic disease , and parainfluenza-3 ( PI-3 ) .
	manualset3
218012	2	420204	7	NULL	NULL	0	NULL	infectious diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Serology for infectious diseases included blue-tongue , brucellosis , bovine respiratory syncytial virus infection , bovine viral diarrhea/mucosal disease , infectious bovine rhinotracheitis , Johne 's disease ( paratuberculosis ) , foot and mouth disease ( FMD ) , leptospirosis ( eight serovars ) , epizootic hemorrhagic disease , and parainfluenza-3 ( PI-3 ) .
	manualset3
218013	3	420204	7	NULL	NULL	0	NULL	blue-tongue	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serology for infectious diseases included blue-tongue , brucellosis , bovine respiratory syncytial virus infection , bovine viral diarrhea/mucosal disease , infectious bovine rhinotracheitis , Johne 's disease ( paratuberculosis ) , foot and mouth disease ( FMD ) , leptospirosis ( eight serovars ) , epizootic hemorrhagic disease , and parainfluenza-3 ( PI-3 ) .
	manualset3
218014	4	420204	7	NULL	NULL	0	NULL	brucellosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Serology for infectious diseases included blue-tongue , brucellosis , bovine respiratory syncytial virus infection , bovine viral diarrhea/mucosal disease , infectious bovine rhinotracheitis , Johne 's disease ( paratuberculosis ) , foot and mouth disease ( FMD ) , leptospirosis ( eight serovars ) , epizootic hemorrhagic disease , and parainfluenza-3 ( PI-3 ) .
	manualset3
218015	5	420204	7	NULL	NULL	0	NULL	bovine respiratory syncytial virus infection	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Serology for infectious diseases included blue-tongue , brucellosis , bovine respiratory syncytial virus infection , bovine viral diarrhea/mucosal disease , infectious bovine rhinotracheitis , Johne 's disease ( paratuberculosis ) , foot and mouth disease ( FMD ) , leptospirosis ( eight serovars ) , epizootic hemorrhagic disease , and parainfluenza-3 ( PI-3 ) .
	manualset3
218016	6	420204	7	NULL	NULL	0	NULL	 bovine viral diarrhea/mucosal disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Serology for infectious diseases included blue-tongue , brucellosis , bovine respiratory syncytial virus infection , bovine viral diarrhea/mucosal disease , infectious bovine rhinotracheitis , Johne 's disease ( paratuberculosis ) , foot and mouth disease ( FMD ) , leptospirosis ( eight serovars ) , epizootic hemorrhagic disease , and parainfluenza-3 ( PI-3 ) .
	manualset3
218017	7	420204	7	NULL	NULL	0	NULL	infectious bovine rhinotracheitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Serology for infectious diseases included blue-tongue , brucellosis , bovine respiratory syncytial virus infection , bovine viral diarrhea/mucosal disease , infectious bovine rhinotracheitis , Johne 's disease ( paratuberculosis ) , foot and mouth disease ( FMD ) , leptospirosis ( eight serovars ) , epizootic hemorrhagic disease , and parainfluenza-3 ( PI-3 ) .
	manualset3
218018	8	420204	7	NULL	NULL	0	NULL	Johne 's disease ( paratuberculosis ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Serology for infectious diseases included blue-tongue , brucellosis , bovine respiratory syncytial virus infection , bovine viral diarrhea/mucosal disease , infectious bovine rhinotracheitis , Johne 's disease ( paratuberculosis ) , foot and mouth disease ( FMD ) , leptospirosis ( eight serovars ) , epizootic hemorrhagic disease , and parainfluenza-3 ( PI-3 ) .
	manualset3
218019	9	420204	7	NULL	NULL	0	NULL	foot and mouth disease ( FMD ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Serology for infectious diseases included blue-tongue , brucellosis , bovine respiratory syncytial virus infection , bovine viral diarrhea/mucosal disease , infectious bovine rhinotracheitis , Johne 's disease ( paratuberculosis ) , foot and mouth disease ( FMD ) , leptospirosis ( eight serovars ) , epizootic hemorrhagic disease , and parainfluenza-3 ( PI-3 ) .
	manualset3
218020	10	420204	7	NULL	NULL	NULL	NULL	leptospirosis 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Serology for infectious diseases included blue-tongue , brucellosis , bovine respiratory syncytial virus infection , bovine viral diarrhea/mucosal disease , infectious bovine rhinotracheitis , Johne 's disease ( paratuberculosis ) , foot and mouth disease ( FMD ) , leptospirosis ( eight serovars ) , epizootic hemorrhagic disease , and parainfluenza-3 ( PI-3 ) .
	manualset3
218021	11	420204	7	NULL	NULL	0	NULL	eight serovars	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Serology for infectious diseases included blue-tongue , brucellosis , bovine respiratory syncytial virus infection , bovine viral diarrhea/mucosal disease , infectious bovine rhinotracheitis , Johne 's disease ( paratuberculosis ) , foot and mouth disease ( FMD ) , leptospirosis ( eight serovars ) , epizootic hemorrhagic disease , and parainfluenza-3 ( PI-3 ) .
	manualset3
218022	12	420204	7	NULL	NULL	0	NULL	epizootic hemorrhagic disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Serology for infectious diseases included blue-tongue , brucellosis , bovine respiratory syncytial virus infection , bovine viral diarrhea/mucosal disease , infectious bovine rhinotracheitis , Johne 's disease ( paratuberculosis ) , foot and mouth disease ( FMD ) , leptospirosis ( eight serovars ) , epizootic hemorrhagic disease , and parainfluenza-3 ( PI-3 ) .
	manualset3
218023	13	420204	7	NULL	NULL	0	NULL	parainfluenza-3 ( PI-3 )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Serology for infectious diseases included blue-tongue , brucellosis , bovine respiratory syncytial virus infection , bovine viral diarrhea/mucosal disease , infectious bovine rhinotracheitis , Johne 's disease ( paratuberculosis ) , foot and mouth disease ( FMD ) , leptospirosis ( eight serovars ) , epizootic hemorrhagic disease , and parainfluenza-3 ( PI-3 ) .
	manualset3
218024	1	420205	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of mercury on vascular smooth muscle results in vasoconstriction , but the mechanism of this action is not elucidated yet .
	manualset3
218025	2	420205	7	NULL	NULL	0	NULL	 mercury	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of mercury on vascular smooth muscle results in vasoconstriction , but the mechanism of this action is not elucidated yet .
	manualset3
218026	3	420205	7	NULL	NULL	0	NULL	vascular smooth muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of mercury on vascular smooth muscle results in vasoconstriction , but the mechanism of this action is not elucidated yet .
	manualset3
218027	4	420205	7	NULL	NULL	0	NULL	vasoconstriction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of mercury on vascular smooth muscle results in vasoconstriction , but the mechanism of this action is not elucidated yet .
	manualset3
218028	5	420205	7	NULL	NULL	0	NULL	 mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of mercury on vascular smooth muscle results in vasoconstriction , but the mechanism of this action is not elucidated yet .
	manualset3
218029	6	420205	7	NULL	NULL	0	NULL	action	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of mercury on vascular smooth muscle results in vasoconstriction , but the mechanism of this action is not elucidated yet .
	manualset3
218030	1	420206	7	NULL	NULL	0	NULL	Chromosomal analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Chromosomal analysis of HSR evolution in situ , by examining individual colonies presumably derived from one or a few cells , underscored this impression of chromosome structural fluidity .
	manualset3
218031	2	420206	7	NULL	NULL	0	NULL	HSR evolution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Chromosomal analysis of HSR evolution in situ , by examining individual colonies presumably derived from one or a few cells , underscored this impression of chromosome structural fluidity .
	manualset3
218032	3	420206	7	NULL	NULL	0	NULL	 individual colonies	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Chromosomal analysis of HSR evolution in situ , by examining individual colonies presumably derived from one or a few cells , underscored this impression of chromosome structural fluidity .
	manualset3
218033	4	420206	7	NULL	NULL	0	NULL	 one 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Chromosomal analysis of HSR evolution in situ , by examining individual colonies presumably derived from one or a few cells , underscored this impression of chromosome structural fluidity .
	manualset3
218034	5	420206	7	NULL	NULL	0	NULL	few cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Chromosomal analysis of HSR evolution in situ , by examining individual colonies presumably derived from one or a few cells , underscored this impression of chromosome structural fluidity .
	manualset3
218035	6	420206	7	NULL	NULL	0	NULL	 impression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Chromosomal analysis of HSR evolution in situ , by examining individual colonies presumably derived from one or a few cells , underscored this impression of chromosome structural fluidity .
	manualset3
218036	7	420206	7	NULL	NULL	0	NULL	chromosome structural fluidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Chromosomal analysis of HSR evolution in situ , by examining individual colonies presumably derived from one or a few cells , underscored this impression of chromosome structural fluidity .
	manualset3
218037	1	420207	7	NULL	NULL	0	NULL	activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , activation of cAMP-dependent protein kinase ( PKA ) by 8-bromo-cAMP caused an inhibition of the L-channel current .
	manualset3
218038	2	420207	7	NULL	NULL	0	NULL	cAMP-dependent protein kinase ( PKA )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , activation of cAMP-dependent protein kinase ( PKA ) by 8-bromo-cAMP caused an inhibition of the L-channel current .
	manualset3
218039	3	420207	7	NULL	NULL	0	NULL	8-bromo-cAMP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , activation of cAMP-dependent protein kinase ( PKA ) by 8-bromo-cAMP caused an inhibition of the L-channel current .
	manualset3
218040	4	420207	7	NULL	NULL	0	NULL	inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , activation of cAMP-dependent protein kinase ( PKA ) by 8-bromo-cAMP caused an inhibition of the L-channel current .
	manualset3
218041	5	420207	7	NULL	NULL	0	NULL	L-channel current	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , activation of cAMP-dependent protein kinase ( PKA ) by 8-bromo-cAMP caused an inhibition of the L-channel current .
	manualset3
218042	1	420208	7	NULL	NULL	0	NULL	25 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We found that 25 % of the CTS patients without confounding neurologic disorders had normal NCS with median palmar nerve stimulation .
	manualset3
218043	2	420208	7	NULL	NULL	0	NULL	CTS patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We found that 25 % of the CTS patients without confounding neurologic disorders had normal NCS with median palmar nerve stimulation .
	manualset3
218044	3	420208	7	NULL	NULL	0	NULL	neurologic disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We found that 25 % of the CTS patients without confounding neurologic disorders had normal NCS with median palmar nerve stimulation .
	manualset3
218045	4	420208	7	NULL	NULL	0	NULL	normal NCS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We found that 25 % of the CTS patients without confounding neurologic disorders had normal NCS with median palmar nerve stimulation .
	manualset3
218046	5	420208	7	NULL	NULL	0	NULL	median palmar nerve stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We found that 25 % of the CTS patients without confounding neurologic disorders had normal NCS with median palmar nerve stimulation .
	manualset3
218047	1	420209	7	NULL	NULL	0	NULL	speculation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there has been much speculation as to its role in clinical transplantation , especially with regard to chronic rejection , indirect T cell allorecognition has been difficult to demonstrate in transplant patients .
	manualset3
218048	2	420209	7	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there has been much speculation as to its role in clinical transplantation , especially with regard to chronic rejection , indirect T cell allorecognition has been difficult to demonstrate in transplant patients .
	manualset3
218049	3	420209	7	NULL	NULL	0	NULL	clinical transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there has been much speculation as to its role in clinical transplantation , especially with regard to chronic rejection , indirect T cell allorecognition has been difficult to demonstrate in transplant patients .
	manualset3
218050	4	420209	7	NULL	NULL	0	NULL	chronic rejection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there has been much speculation as to its role in clinical transplantation , especially with regard to chronic rejection , indirect T cell allorecognition has been difficult to demonstrate in transplant patients .
	manualset3
218051	5	420209	7	NULL	NULL	0	NULL	indirect T cell allorecognition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there has been much speculation as to its role in clinical transplantation , especially with regard to chronic rejection , indirect T cell allorecognition has been difficult to demonstrate in transplant patients .
	manualset3
218052	6	420209	7	NULL	NULL	0	NULL	transplant patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there has been much speculation as to its role in clinical transplantation , especially with regard to chronic rejection , indirect T cell allorecognition has been difficult to demonstrate in transplant patients .
	manualset3
218053	1	420210	7	NULL	NULL	0	NULL	Nickel-catalyzed borylative ring opening	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nickel-catalyzed borylative ring opening of vinyl epoxides and aziridines .
	manualset3
218054	2	420210	7	NULL	NULL	0	NULL	vinyl epoxides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nickel-catalyzed borylative ring opening of vinyl epoxides and aziridines .
	manualset3
218055	3	420210	7	NULL	NULL	0	NULL	aziridines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nickel-catalyzed borylative ring opening of vinyl epoxides and aziridines .
	manualset3
218056	1	420211	7	NULL	NULL	0	NULL	International patent barriers	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	International patent barriers will be a crucial step to move the whole stem cell research community forward .
	manualset3
218057	2	420211	7	NULL	NULL	0	NULL	crucial step 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	International patent barriers will be a crucial step to move the whole stem cell research community forward .
	manualset3
218058	3	420211	7	NULL	NULL	0	NULL	whole stem cell research community	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	International patent barriers will be a crucial step to move the whole stem cell research community forward .
	manualset3
218059	1	420212	7	NULL	NULL	0	NULL	amidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This amidase hydrolyzed propionamide efficiently , and also hydrolyzed , at a lower efficiency , acetamide , acrylamide and indoleacetamide .
	manualset3
218060	2	420212	7	NULL	NULL	0	NULL	propionamide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This amidase hydrolyzed propionamide efficiently , and also hydrolyzed , at a lower efficiency , acetamide , acrylamide and indoleacetamide .
	manualset3
218061	3	420212	7	NULL	NULL	0	NULL	lower efficiency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This amidase hydrolyzed propionamide efficiently , and also hydrolyzed , at a lower efficiency , acetamide , acrylamide and indoleacetamide .
	manualset3
218062	4	420212	7	NULL	NULL	0	NULL	acetamide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This amidase hydrolyzed propionamide efficiently , and also hydrolyzed , at a lower efficiency , acetamide , acrylamide and indoleacetamide .
	manualset3
218063	5	420212	7	NULL	NULL	0	NULL	acrylamide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This amidase hydrolyzed propionamide efficiently , and also hydrolyzed , at a lower efficiency , acetamide , acrylamide and indoleacetamide .
	manualset3
218064	6	420212	7	NULL	NULL	0	NULL	indoleacetamide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This amidase hydrolyzed propionamide efficiently , and also hydrolyzed , at a lower efficiency , acetamide , acrylamide and indoleacetamide .
	manualset3
218065	1	420213	7	NULL	NULL	0	NULL	Introduced cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Introduced cases of cutaneous leishmaniasis in Egypt .
	manualset3
218066	2	420213	7	NULL	NULL	0	NULL	cutaneous leishmaniasis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Introduced cases of cutaneous leishmaniasis in Egypt .
	manualset3
218067	3	420213	7	NULL	NULL	0	NULL	Egypt	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Introduced cases of cutaneous leishmaniasis in Egypt .
	manualset3
218068	1	420214	7	NULL	NULL	0	NULL	JCAHO undercutting role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	JCAHO undercutting role of safety management , life safety .
	manualset3
218069	2	420214	7	NULL	NULL	0	NULL	safety management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	JCAHO undercutting role of safety management , life safety .
	manualset3
218070	3	420214	7	NULL	NULL	NULL	NULL	 life safety	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	JCAHO undercutting role of safety management , life safety .
	manualset3
218071	1	420215	7	NULL	NULL	0	NULL	mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mutation of Trp59 or Phe99 generates an FKBP12 with a significantly lower affinity for FK506 than wild-type protein .
	manualset3
218072	2	420215	7	NULL	NULL	0	NULL	Trp59	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The mutation of Trp59 or Phe99 generates an FKBP12 with a significantly lower affinity for FK506 than wild-type protein .
	manualset3
218073	3	420215	7	NULL	NULL	0	NULL	Phe99	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The mutation of Trp59 or Phe99 generates an FKBP12 with a significantly lower affinity for FK506 than wild-type protein .
	manualset3
218074	4	420215	7	NULL	NULL	0	NULL	FKBP12	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mutation of Trp59 or Phe99 generates an FKBP12 with a significantly lower affinity for FK506 than wild-type protein .
	manualset3
218075	5	420215	7	NULL	NULL	0	NULL	lower affinity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mutation of Trp59 or Phe99 generates an FKBP12 with a significantly lower affinity for FK506 than wild-type protein .
	manualset3
218076	6	420215	7	NULL	NULL	0	NULL	FK506	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mutation of Trp59 or Phe99 generates an FKBP12 with a significantly lower affinity for FK506 than wild-type protein .
	manualset3
218077	7	420215	7	NULL	NULL	0	NULL	wild-type protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mutation of Trp59 or Phe99 generates an FKBP12 with a significantly lower affinity for FK506 than wild-type protein .
	manualset3
218078	1	420216	7	NULL	NULL	0	NULL	Mammalian nuclear DNA polymerases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mammalian nuclear DNA polymerases alpha and beta are lack of the proofreading 3 ' -- ) 5 ' exonucleolytic activity .
	manualset3
218079	2	420216	7	NULL	NULL	0	NULL	alpha	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mammalian nuclear DNA polymerases alpha and beta are lack of the proofreading 3 ' -- ) 5 ' exonucleolytic activity .
	manualset3
218080	3	420216	7	NULL	NULL	0	NULL	beta 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mammalian nuclear DNA polymerases alpha and beta are lack of the proofreading 3 ' -- ) 5 ' exonucleolytic activity .
	manualset3
218081	4	420216	7	NULL	NULL	0	NULL	proofreading 3 ' -- ) 5 ' exonucleolytic activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mammalian nuclear DNA polymerases alpha and beta are lack of the proofreading 3 ' -- ) 5 ' exonucleolytic activity .
	manualset3
218082	1	420217	7	NULL	NULL	0	NULL	no change	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there was no change in serum cholesterol levels ( total , LDL , or high-density lipoprotein ) , serum lipid peroxidation and LDL oxidation were significantly decreased .
	manualset3
218083	2	420217	7	NULL	NULL	0	NULL	serum cholesterol levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there was no change in serum cholesterol levels ( total , LDL , or high-density lipoprotein ) , serum lipid peroxidation and LDL oxidation were significantly decreased .
	manualset3
218084	3	420217	7	NULL	NULL	NULL	NULL	total lipoprotein	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although there was no change in serum cholesterol levels ( total , LDL , or high-density lipoprotein ) , serum lipid peroxidation and LDL oxidation were significantly decreased .
	manualset3
218085	4	420217	7	NULL	NULL	0	NULL	LDL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there was no change in serum cholesterol levels ( total , LDL , or high-density lipoprotein ) , serum lipid peroxidation and LDL oxidation were significantly decreased .
	manualset3
218086	5	420217	7	NULL	NULL	0	NULL	high-density lipoprotein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there was no change in serum cholesterol levels ( total , LDL , or high-density lipoprotein ) , serum lipid peroxidation and LDL oxidation were significantly decreased .
	manualset3
218087	6	420217	7	NULL	NULL	0	NULL	serum lipid peroxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there was no change in serum cholesterol levels ( total , LDL , or high-density lipoprotein ) , serum lipid peroxidation and LDL oxidation were significantly decreased .
	manualset3
218088	7	420217	7	NULL	NULL	0	NULL	LDL oxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there was no change in serum cholesterol levels ( total , LDL , or high-density lipoprotein ) , serum lipid peroxidation and LDL oxidation were significantly decreased .
	manualset3
218089	1	420218	7	NULL	NULL	0	NULL	Trypanosoma cruzi	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Trypanosoma cruzi : Oxidative stress induces arginine kinase expression .
	manualset3
218090	2	420218	7	NULL	NULL	0	NULL	Oxidative stress	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Trypanosoma cruzi : Oxidative stress induces arginine kinase expression .
	manualset3
218091	3	420218	7	NULL	NULL	0	NULL	arginine kinase expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Trypanosoma cruzi : Oxidative stress induces arginine kinase expression .
	manualset3
218092	1	420219	7	NULL	NULL	0	NULL	JP patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All JP patients displayed intrinsic cell defects in chemotaxis compared with controls ; in addition , some patients displayed multiple defects , including those which were serum-associated .
	manualset3
218093	2	420219	7	NULL	NULL	0	NULL	intrinsic cell defects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All JP patients displayed intrinsic cell defects in chemotaxis compared with controls ; in addition , some patients displayed multiple defects , including those which were serum-associated .
	manualset3
218094	3	420219	7	NULL	NULL	0	NULL	chemotaxis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All JP patients displayed intrinsic cell defects in chemotaxis compared with controls ; in addition , some patients displayed multiple defects , including those which were serum-associated .
	manualset3
218095	4	420219	7	NULL	NULL	0	NULL	controls	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	All JP patients displayed intrinsic cell defects in chemotaxis compared with controls ; in addition , some patients displayed multiple defects , including those which were serum-associated .
	manualset3
218096	5	420219	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	All JP patients displayed intrinsic cell defects in chemotaxis compared with controls ; in addition , some patients displayed multiple defects , including those which were serum-associated .
	manualset3
218097	6	420219	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All JP patients displayed intrinsic cell defects in chemotaxis compared with controls ; in addition , some patients displayed multiple defects , including those which were serum-associated .
	manualset3
218098	7	420219	7	NULL	NULL	0	NULL	multiple defects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All JP patients displayed intrinsic cell defects in chemotaxis compared with controls ; in addition , some patients displayed multiple defects , including those which were serum-associated .
	manualset3
218099	1	420220	7	NULL	NULL	0	NULL	Cellulitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Cellulitis and spondylitis due to Streptococcus pneumoniae .
	manualset3
218100	2	420220	7	NULL	NULL	0	NULL	 spondylitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Cellulitis and spondylitis due to Streptococcus pneumoniae .
	manualset3
218101	3	420220	7	NULL	NULL	0	NULL	Streptococcus pneumoniae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Cellulitis and spondylitis due to Streptococcus pneumoniae .
	manualset3
218102	1	420221	7	NULL	NULL	0	NULL	80 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , 80 % of sick people in developing countries have a water related illness , be it transmitted by contaminated water or by insects and snails that reproduce in the water .
	manualset3
218103	2	420221	7	NULL	NULL	0	NULL	 sick people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , 80 % of sick people in developing countries have a water related illness , be it transmitted by contaminated water or by insects and snails that reproduce in the water .
	manualset3
218104	3	420221	7	NULL	NULL	0	NULL	developing countries	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , 80 % of sick people in developing countries have a water related illness , be it transmitted by contaminated water or by insects and snails that reproduce in the water .
	manualset3
218105	4	420221	7	NULL	NULL	0	NULL	water related illness	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , 80 % of sick people in developing countries have a water related illness , be it transmitted by contaminated water or by insects and snails that reproduce in the water .
	manualset3
218106	5	420221	7	NULL	NULL	0	NULL	contaminated water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , 80 % of sick people in developing countries have a water related illness , be it transmitted by contaminated water or by insects and snails that reproduce in the water .
	manualset3
218107	6	420221	7	NULL	NULL	0	NULL	insects 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , 80 % of sick people in developing countries have a water related illness , be it transmitted by contaminated water or by insects and snails that reproduce in the water .
	manualset3
218108	7	420221	7	NULL	NULL	0	NULL	snails	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , 80 % of sick people in developing countries have a water related illness , be it transmitted by contaminated water or by insects and snails that reproduce in the water .
	manualset3
218109	8	420221	7	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , 80 % of sick people in developing countries have a water related illness , be it transmitted by contaminated water or by insects and snails that reproduce in the water .
	manualset3
218110	1	420222	7	NULL	NULL	0	NULL	Secondary structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Secondary structure of human interleukin 2 from 3D heteronuclear NMR experiments .
	manualset3
218111	2	420222	7	NULL	NULL	0	NULL	human interleukin 2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Secondary structure of human interleukin 2 from 3D heteronuclear NMR experiments .
	manualset3
218112	3	420222	7	NULL	NULL	0	NULL	 3D heteronuclear NMR experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Secondary structure of human interleukin 2 from 3D heteronuclear NMR experiments .
	manualset3
218113	1	420223	7	NULL	NULL	0	NULL	no difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there was no difference between groups in LV weight or infarct size measured upon necropsy , there was a dramatic reduction in RV hypertrophy and lung congestion ( decrease of 22-48 % , P & lt ; 0.01 ) with treatment which was associated with a ) 7-fold decrease ( P & lt ; 0.05 ) in aterial natriuretic peptide gene expression in RV .
	manualset3
218114	2	420223	7	NULL	NULL	0	NULL	groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there was no difference between groups in LV weight or infarct size measured upon necropsy , there was a dramatic reduction in RV hypertrophy and lung congestion ( decrease of 22-48 % , P & lt ; 0.01 ) with treatment which was associated with a ) 7-fold decrease ( P & lt ; 0.05 ) in aterial natriuretic peptide gene expression in RV .
	manualset3
218115	3	420223	7	NULL	NULL	0	NULL	LV weight 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there was no difference between groups in LV weight or infarct size measured upon necropsy , there was a dramatic reduction in RV hypertrophy and lung congestion ( decrease of 22-48 % , P & lt ; 0.01 ) with treatment which was associated with a ) 7-fold decrease ( P & lt ; 0.05 ) in aterial natriuretic peptide gene expression in RV .
	manualset3
218116	4	420223	7	NULL	NULL	0	NULL	infarct size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there was no difference between groups in LV weight or infarct size measured upon necropsy , there was a dramatic reduction in RV hypertrophy and lung congestion ( decrease of 22-48 % , P & lt ; 0.01 ) with treatment which was associated with a ) 7-fold decrease ( P & lt ; 0.05 ) in aterial natriuretic peptide gene expression in RV .
	manualset3
218117	5	420223	7	NULL	NULL	0	NULL	necropsy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there was no difference between groups in LV weight or infarct size measured upon necropsy , there was a dramatic reduction in RV hypertrophy and lung congestion ( decrease of 22-48 % , P & lt ; 0.01 ) with treatment which was associated with a ) 7-fold decrease ( P & lt ; 0.05 ) in aterial natriuretic peptide gene expression in RV .
	manualset3
218118	6	420223	7	NULL	NULL	0	NULL	dramatic reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there was no difference between groups in LV weight or infarct size measured upon necropsy , there was a dramatic reduction in RV hypertrophy and lung congestion ( decrease of 22-48 % , P & lt ; 0.01 ) with treatment which was associated with a ) 7-fold decrease ( P & lt ; 0.05 ) in aterial natriuretic peptide gene expression in RV .
	manualset3
218119	7	420223	7	NULL	NULL	0	NULL	RV hypertrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there was no difference between groups in LV weight or infarct size measured upon necropsy , there was a dramatic reduction in RV hypertrophy and lung congestion ( decrease of 22-48 % , P & lt ; 0.01 ) with treatment which was associated with a ) 7-fold decrease ( P & lt ; 0.05 ) in aterial natriuretic peptide gene expression in RV .
	manualset3
218120	8	420223	7	NULL	NULL	0	NULL	lung congestion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there was no difference between groups in LV weight or infarct size measured upon necropsy , there was a dramatic reduction in RV hypertrophy and lung congestion ( decrease of 22-48 % , P & lt ; 0.01 ) with treatment which was associated with a ) 7-fold decrease ( P & lt ; 0.05 ) in aterial natriuretic peptide gene expression in RV .
	manualset3
218121	9	420223	7	NULL	NULL	0	NULL	decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there was no difference between groups in LV weight or infarct size measured upon necropsy , there was a dramatic reduction in RV hypertrophy and lung congestion ( decrease of 22-48 % , P & lt ; 0.01 ) with treatment which was associated with a ) 7-fold decrease ( P & lt ; 0.05 ) in aterial natriuretic peptide gene expression in RV .
	manualset3
218122	10	420223	7	NULL	NULL	0	NULL	22-48 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there was no difference between groups in LV weight or infarct size measured upon necropsy , there was a dramatic reduction in RV hypertrophy and lung congestion ( decrease of 22-48 % , P & lt ; 0.01 ) with treatment which was associated with a ) 7-fold decrease ( P & lt ; 0.05 ) in aterial natriuretic peptide gene expression in RV .
	manualset3
218123	11	420223	7	NULL	NULL	0	NULL	P & lt ; 0.01	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there was no difference between groups in LV weight or infarct size measured upon necropsy , there was a dramatic reduction in RV hypertrophy and lung congestion ( decrease of 22-48 % , P & lt ; 0.01 ) with treatment which was associated with a ) 7-fold decrease ( P & lt ; 0.05 ) in aterial natriuretic peptide gene expression in RV .
	manualset3
218124	12	420223	7	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there was no difference between groups in LV weight or infarct size measured upon necropsy , there was a dramatic reduction in RV hypertrophy and lung congestion ( decrease of 22-48 % , P & lt ; 0.01 ) with treatment which was associated with a ) 7-fold decrease ( P & lt ; 0.05 ) in aterial natriuretic peptide gene expression in RV .
	manualset3
218125	13	420223	7	NULL	NULL	0	NULL	7-fold decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there was no difference between groups in LV weight or infarct size measured upon necropsy , there was a dramatic reduction in RV hypertrophy and lung congestion ( decrease of 22-48 % , P & lt ; 0.01 ) with treatment which was associated with a ) 7-fold decrease ( P & lt ; 0.05 ) in aterial natriuretic peptide gene expression in RV .
	manualset3
218126	14	420223	7	NULL	NULL	0	NULL	P & lt ; 0.05	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there was no difference between groups in LV weight or infarct size measured upon necropsy , there was a dramatic reduction in RV hypertrophy and lung congestion ( decrease of 22-48 % , P & lt ; 0.01 ) with treatment which was associated with a ) 7-fold decrease ( P & lt ; 0.05 ) in aterial natriuretic peptide gene expression in RV .
	manualset3
218127	15	420223	7	NULL	NULL	0	NULL	aterial natriuretic peptide gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there was no difference between groups in LV weight or infarct size measured upon necropsy , there was a dramatic reduction in RV hypertrophy and lung congestion ( decrease of 22-48 % , P & lt ; 0.01 ) with treatment which was associated with a ) 7-fold decrease ( P & lt ; 0.05 ) in aterial natriuretic peptide gene expression in RV .
	manualset3
218128	16	420223	7	NULL	NULL	0	NULL	RV	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there was no difference between groups in LV weight or infarct size measured upon necropsy , there was a dramatic reduction in RV hypertrophy and lung congestion ( decrease of 22-48 % , P & lt ; 0.01 ) with treatment which was associated with a ) 7-fold decrease ( P & lt ; 0.05 ) in aterial natriuretic peptide gene expression in RV .
	manualset3
218129	1	420224	7	NULL	NULL	0	NULL	Rp-8-Br-PET-cGMPS	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Rp-8-Br-PET-cGMPS inhibited OT release at 1 nM .
	manualset3
218130	2	420224	7	NULL	NULL	0	NULL	OT release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rp-8-Br-PET-cGMPS inhibited OT release at 1 nM .
	manualset3
218131	3	420224	7	NULL	NULL	0	NULL	 1 nM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Rp-8-Br-PET-cGMPS inhibited OT release at 1 nM .
	manualset3
218132	1	420225	7	NULL	NULL	NULL	NULL	Subunit folding	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Subunit folding and processing continue with formation of the ligand-binding sites on the alpha subunit of alphabetagammadelta tetramers and the second alpha subunit added to assemble alpha ( 2 ) betagammadelta pentamers .
	manualset3
218133	2	420225	7	NULL	NULL	NULL	NULL	processing	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Subunit folding and processing continue with formation of the ligand-binding sites on the alpha subunit of alphabetagammadelta tetramers and the second alpha subunit added to assemble alpha ( 2 ) betagammadelta pentamers .
	manualset3
218134	3	420225	7	NULL	NULL	0	NULL	formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subunit folding and processing continue with formation of the ligand-binding sites on the alpha subunit of alphabetagammadelta tetramers and the second alpha subunit added to assemble alpha ( 2 ) betagammadelta pentamers .
	manualset3
218135	4	420225	7	NULL	NULL	0	NULL	ligand-binding sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Subunit folding and processing continue with formation of the ligand-binding sites on the alpha subunit of alphabetagammadelta tetramers and the second alpha subunit added to assemble alpha ( 2 ) betagammadelta pentamers .
	manualset3
218136	5	420225	7	NULL	NULL	0	NULL	 alpha subunit	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Subunit folding and processing continue with formation of the ligand-binding sites on the alpha subunit of alphabetagammadelta tetramers and the second alpha subunit added to assemble alpha ( 2 ) betagammadelta pentamers .
	manualset3
218137	6	420225	7	NULL	NULL	0	NULL	alphabetagammadelta tetramers	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Subunit folding and processing continue with formation of the ligand-binding sites on the alpha subunit of alphabetagammadelta tetramers and the second alpha subunit added to assemble alpha ( 2 ) betagammadelta pentamers .
	manualset3
218138	7	420225	7	NULL	NULL	0	NULL	second alpha subunit	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Subunit folding and processing continue with formation of the ligand-binding sites on the alpha subunit of alphabetagammadelta tetramers and the second alpha subunit added to assemble alpha ( 2 ) betagammadelta pentamers .
	manualset3
218139	8	420225	7	NULL	NULL	0	NULL	alpha ( 2 ) betagammadelta pentamers	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Subunit folding and processing continue with formation of the ligand-binding sites on the alpha subunit of alphabetagammadelta tetramers and the second alpha subunit added to assemble alpha ( 2 ) betagammadelta pentamers .
	manualset3
218140	1	420226	7	NULL	NULL	0	NULL	previous study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous study , we demonstrated that androgenic-anabolic steroids increased aromatase expression in the bed nucleus of stria terminalis and preoptic area in rat brain , as evaluated using autoradiography with ( 11C ) vorozole , a potential positron emission tomography tracer for aromatase .
	manualset3
218141	2	420226	7	NULL	NULL	0	NULL	androgenic-anabolic steroids	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous study , we demonstrated that androgenic-anabolic steroids increased aromatase expression in the bed nucleus of stria terminalis and preoptic area in rat brain , as evaluated using autoradiography with ( 11C ) vorozole , a potential positron emission tomography tracer for aromatase .
	manualset3
218142	3	420226	7	NULL	NULL	0	NULL	aromatase expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous study , we demonstrated that androgenic-anabolic steroids increased aromatase expression in the bed nucleus of stria terminalis and preoptic area in rat brain , as evaluated using autoradiography with ( 11C ) vorozole , a potential positron emission tomography tracer for aromatase .
	manualset3
218143	4	420226	7	NULL	NULL	0	NULL	bed nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous study , we demonstrated that androgenic-anabolic steroids increased aromatase expression in the bed nucleus of stria terminalis and preoptic area in rat brain , as evaluated using autoradiography with ( 11C ) vorozole , a potential positron emission tomography tracer for aromatase .
	manualset3
218144	5	420226	7	NULL	NULL	NULL	NULL	stria terminalis	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In a previous study , we demonstrated that androgenic-anabolic steroids increased aromatase expression in the bed nucleus of stria terminalis and preoptic area in rat brain , as evaluated using autoradiography with ( 11C ) vorozole , a potential positron emission tomography tracer for aromatase .
	manualset3
218145	6	420226	7	NULL	NULL	0	NULL	preoptic area	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous study , we demonstrated that androgenic-anabolic steroids increased aromatase expression in the bed nucleus of stria terminalis and preoptic area in rat brain , as evaluated using autoradiography with ( 11C ) vorozole , a potential positron emission tomography tracer for aromatase .
	manualset3
218146	7	420226	7	NULL	NULL	0	NULL	rat brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous study , we demonstrated that androgenic-anabolic steroids increased aromatase expression in the bed nucleus of stria terminalis and preoptic area in rat brain , as evaluated using autoradiography with ( 11C ) vorozole , a potential positron emission tomography tracer for aromatase .
	manualset3
218147	8	420226	7	NULL	NULL	0	NULL	autoradiography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous study , we demonstrated that androgenic-anabolic steroids increased aromatase expression in the bed nucleus of stria terminalis and preoptic area in rat brain , as evaluated using autoradiography with ( 11C ) vorozole , a potential positron emission tomography tracer for aromatase .
	manualset3
218148	9	420226	7	NULL	NULL	0	NULL	( 11C ) vorozole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous study , we demonstrated that androgenic-anabolic steroids increased aromatase expression in the bed nucleus of stria terminalis and preoptic area in rat brain , as evaluated using autoradiography with ( 11C ) vorozole , a potential positron emission tomography tracer for aromatase .
	manualset3
218149	10	420226	7	NULL	NULL	0	NULL	potential positron emission tomography tracer	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous study , we demonstrated that androgenic-anabolic steroids increased aromatase expression in the bed nucleus of stria terminalis and preoptic area in rat brain , as evaluated using autoradiography with ( 11C ) vorozole , a potential positron emission tomography tracer for aromatase .
	manualset3
218150	11	420226	7	NULL	NULL	0	NULL	aromatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In a previous study , we demonstrated that androgenic-anabolic steroids increased aromatase expression in the bed nucleus of stria terminalis and preoptic area in rat brain , as evaluated using autoradiography with ( 11C ) vorozole , a potential positron emission tomography tracer for aromatase .
	manualset3
218151	1	420227	7	NULL	NULL	0	NULL	268	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	268 of tumors were histologically verified ( 73.8 % ) and 95 of cases were evaluated according to the neurosurgeon 's point of view and/or to the clinical and CT controls ( 26.2 % ) , because of the biopsy ( especially in the pre-CT era ) was highly riskfull .
	manualset3
218152	2	420227	7	NULL	NULL	0	NULL	tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	268 of tumors were histologically verified ( 73.8 % ) and 95 of cases were evaluated according to the neurosurgeon 's point of view and/or to the clinical and CT controls ( 26.2 % ) , because of the biopsy ( especially in the pre-CT era ) was highly riskfull .
	manualset3
218153	3	420227	7	NULL	NULL	0	NULL	73.8 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	268 of tumors were histologically verified ( 73.8 % ) and 95 of cases were evaluated according to the neurosurgeon 's point of view and/or to the clinical and CT controls ( 26.2 % ) , because of the biopsy ( especially in the pre-CT era ) was highly riskfull .
	manualset3
218154	4	420227	7	NULL	NULL	0	NULL	95 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	268 of tumors were histologically verified ( 73.8 % ) and 95 of cases were evaluated according to the neurosurgeon 's point of view and/or to the clinical and CT controls ( 26.2 % ) , because of the biopsy ( especially in the pre-CT era ) was highly riskfull .
	manualset3
218155	5	420227	7	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	268 of tumors were histologically verified ( 73.8 % ) and 95 of cases were evaluated according to the neurosurgeon 's point of view and/or to the clinical and CT controls ( 26.2 % ) , because of the biopsy ( especially in the pre-CT era ) was highly riskfull .
	manualset3
218156	6	420227	7	NULL	NULL	0	NULL	neurosurgeon 's point of view	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	268 of tumors were histologically verified ( 73.8 % ) and 95 of cases were evaluated according to the neurosurgeon 's point of view and/or to the clinical and CT controls ( 26.2 % ) , because of the biopsy ( especially in the pre-CT era ) was highly riskfull .
	manualset3
218157	7	420227	7	NULL	NULL	0	NULL	 clinical controls	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	268 of tumors were histologically verified ( 73.8 % ) and 95 of cases were evaluated according to the neurosurgeon 's point of view and/or to the clinical and CT controls ( 26.2 % ) , because of the biopsy ( especially in the pre-CT era ) was highly riskfull .
	manualset3
218158	8	420227	7	NULL	NULL	0	NULL	CT controls 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	268 of tumors were histologically verified ( 73.8 % ) and 95 of cases were evaluated according to the neurosurgeon 's point of view and/or to the clinical and CT controls ( 26.2 % ) , because of the biopsy ( especially in the pre-CT era ) was highly riskfull .
	manualset3
218159	9	420227	7	NULL	NULL	0	NULL	26.2 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	268 of tumors were histologically verified ( 73.8 % ) and 95 of cases were evaluated according to the neurosurgeon 's point of view and/or to the clinical and CT controls ( 26.2 % ) , because of the biopsy ( especially in the pre-CT era ) was highly riskfull .
	manualset3
218160	10	420227	7	NULL	NULL	0	NULL	biopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	268 of tumors were histologically verified ( 73.8 % ) and 95 of cases were evaluated according to the neurosurgeon 's point of view and/or to the clinical and CT controls ( 26.2 % ) , because of the biopsy ( especially in the pre-CT era ) was highly riskfull .
	manualset3
218161	11	420227	7	NULL	NULL	0	NULL	pre-CT era	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	268 of tumors were histologically verified ( 73.8 % ) and 95 of cases were evaluated according to the neurosurgeon 's point of view and/or to the clinical and CT controls ( 26.2 % ) , because of the biopsy ( especially in the pre-CT era ) was highly riskfull .
	manualset3
218162	12	420227	7	NULL	NULL	0	NULL	riskfull	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	268 of tumors were histologically verified ( 73.8 % ) and 95 of cases were evaluated according to the neurosurgeon 's point of view and/or to the clinical and CT controls ( 26.2 % ) , because of the biopsy ( especially in the pre-CT era ) was highly riskfull .
	manualset3
218163	1	420228	7	NULL	NULL	0	NULL	Cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cell proliferation and delayed-type skin reaction induced by soluble toxoplasma tachyzoite antigen followed the same pattern .
	manualset3
218164	2	420228	7	NULL	NULL	0	NULL	delayed-type skin reaction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Cell proliferation and delayed-type skin reaction induced by soluble toxoplasma tachyzoite antigen followed the same pattern .
	manualset3
218165	3	420228	7	NULL	NULL	0	NULL	soluble toxoplasma tachyzoite antigen	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Cell proliferation and delayed-type skin reaction induced by soluble toxoplasma tachyzoite antigen followed the same pattern .
	manualset3
218166	4	420228	7	NULL	NULL	0	NULL	same pattern	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Cell proliferation and delayed-type skin reaction induced by soluble toxoplasma tachyzoite antigen followed the same pattern .
	manualset3
218167	1	420229	7	NULL	NULL	0	NULL	nonobese maturity-onset diabetic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Three nonobese maturity-onset diabetic patients has worsening hyperglycemia and ketonuria unresponsive to marked increases in dose of beef/pork insulin .
	manualset3
218168	2	420229	7	NULL	NULL	0	NULL	hyperglycemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Three nonobese maturity-onset diabetic patients has worsening hyperglycemia and ketonuria unresponsive to marked increases in dose of beef/pork insulin .
	manualset3
218169	3	420229	7	NULL	NULL	0	NULL	ketonuria	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Three nonobese maturity-onset diabetic patients has worsening hyperglycemia and ketonuria unresponsive to marked increases in dose of beef/pork insulin .
	manualset3
218170	4	420229	7	NULL	NULL	0	NULL	increases in dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Three nonobese maturity-onset diabetic patients has worsening hyperglycemia and ketonuria unresponsive to marked increases in dose of beef/pork insulin .
	manualset3
218171	5	420229	7	NULL	NULL	0	NULL	beef/pork insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Three nonobese maturity-onset diabetic patients has worsening hyperglycemia and ketonuria unresponsive to marked increases in dose of beef/pork insulin .
	manualset3
218172	1	420230	7	NULL	NULL	0	NULL	rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In rat , SOM-LI fibers were scattered throughout the AP while moderate accumulations of SOM-LI fibers occurred near the ventrolateral border .
	manualset3
218173	2	420230	7	NULL	NULL	0	NULL	SOM-LI fibers 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In rat , SOM-LI fibers were scattered throughout the AP while moderate accumulations of SOM-LI fibers occurred near the ventrolateral border .
	manualset3
218174	3	420230	7	NULL	NULL	0	NULL	AP	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In rat , SOM-LI fibers were scattered throughout the AP while moderate accumulations of SOM-LI fibers occurred near the ventrolateral border .
	manualset3
218175	4	420230	7	NULL	NULL	0	NULL	accumulations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In rat , SOM-LI fibers were scattered throughout the AP while moderate accumulations of SOM-LI fibers occurred near the ventrolateral border .
	manualset3
218176	5	420230	7	NULL	NULL	0	NULL	SOM-LI fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In rat , SOM-LI fibers were scattered throughout the AP while moderate accumulations of SOM-LI fibers occurred near the ventrolateral border .
	manualset3
218177	6	420230	7	NULL	NULL	0	NULL	ventrolateral border	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In rat , SOM-LI fibers were scattered throughout the AP while moderate accumulations of SOM-LI fibers occurred near the ventrolateral border .
	manualset3
218215	1	420231	7	NULL	NULL	0	NULL	ATMP - Regulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An appropriate ATMP - Regulation is dealing with ATMP requirements .
	manualset3
218216	2	420231	7	NULL	NULL	0	NULL	ATMP requirements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An appropriate ATMP - Regulation is dealing with ATMP requirements .
	manualset3
218217	1	420232	7	NULL	NULL	0	NULL	paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , the paper considers how education in Dental Public Health could be developed to provide more flexible training whilst ensuring that the quality of knowledge and skills of specialists is maintained or improved .
	manualset3
218218	2	420232	7	NULL	NULL	0	NULL	 education 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , the paper considers how education in Dental Public Health could be developed to provide more flexible training whilst ensuring that the quality of knowledge and skills of specialists is maintained or improved .
	manualset3
218219	3	420232	7	NULL	NULL	0	NULL	Dental Public Health	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , the paper considers how education in Dental Public Health could be developed to provide more flexible training whilst ensuring that the quality of knowledge and skills of specialists is maintained or improved .
	manualset3
218220	4	420232	7	NULL	NULL	0	NULL	flexible training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , the paper considers how education in Dental Public Health could be developed to provide more flexible training whilst ensuring that the quality of knowledge and skills of specialists is maintained or improved .
	manualset3
218221	5	420232	7	NULL	NULL	0	NULL	quality	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , the paper considers how education in Dental Public Health could be developed to provide more flexible training whilst ensuring that the quality of knowledge and skills of specialists is maintained or improved .
	manualset3
218222	6	420232	7	NULL	NULL	0	NULL	knowledge	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , the paper considers how education in Dental Public Health could be developed to provide more flexible training whilst ensuring that the quality of knowledge and skills of specialists is maintained or improved .
	manualset3
218223	7	420232	7	NULL	NULL	0	NULL	skills	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , the paper considers how education in Dental Public Health could be developed to provide more flexible training whilst ensuring that the quality of knowledge and skills of specialists is maintained or improved .
	manualset3
218224	8	420232	7	NULL	NULL	0	NULL	specialists 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , the paper considers how education in Dental Public Health could be developed to provide more flexible training whilst ensuring that the quality of knowledge and skills of specialists is maintained or improved .
	manualset3
218225	1	420233	7	NULL	NULL	0	NULL	1.2 fewer pulses	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there were 1.2 fewer pulses during E2 infusion compared to saline infusion , differences did not reach significance ( P = 0.1 ; 95 % confidence interval for the difference , -3.5 , 1.1 ) .
	manualset3
218226	2	420233	7	NULL	NULL	0	NULL	E2 infusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there were 1.2 fewer pulses during E2 infusion compared to saline infusion , differences did not reach significance ( P = 0.1 ; 95 % confidence interval for the difference , -3.5 , 1.1 ) .
	manualset3
218227	3	420233	7	NULL	NULL	0	NULL	saline infusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there were 1.2 fewer pulses during E2 infusion compared to saline infusion , differences did not reach significance ( P = 0.1 ; 95 % confidence interval for the difference , -3.5 , 1.1 ) .
	manualset3
218228	4	420233	7	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there were 1.2 fewer pulses during E2 infusion compared to saline infusion , differences did not reach significance ( P = 0.1 ; 95 % confidence interval for the difference , -3.5 , 1.1 ) .
	manualset3
218229	5	420233	7	NULL	NULL	0	NULL	P = 0.1	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there were 1.2 fewer pulses during E2 infusion compared to saline infusion , differences did not reach significance ( P = 0.1 ; 95 % confidence interval for the difference , -3.5 , 1.1 ) .
	manualset3
218230	6	420233	7	NULL	NULL	0	NULL	95 % confidence interval 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there were 1.2 fewer pulses during E2 infusion compared to saline infusion , differences did not reach significance ( P = 0.1 ; 95 % confidence interval for the difference , -3.5 , 1.1 ) .
	manualset3
218231	7	420233	7	NULL	NULL	0	NULL	difference 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there were 1.2 fewer pulses during E2 infusion compared to saline infusion , differences did not reach significance ( P = 0.1 ; 95 % confidence interval for the difference , -3.5 , 1.1 ) .
	manualset3
218232	8	420233	7	NULL	NULL	0	NULL	 -3.5 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there were 1.2 fewer pulses during E2 infusion compared to saline infusion , differences did not reach significance ( P = 0.1 ; 95 % confidence interval for the difference , -3.5 , 1.1 ) .
	manualset3
218233	9	420233	7	NULL	NULL	0	NULL	 1.1 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there were 1.2 fewer pulses during E2 infusion compared to saline infusion , differences did not reach significance ( P = 0.1 ; 95 % confidence interval for the difference , -3.5 , 1.1 ) .
	manualset3
218234	1	420234	7	NULL	NULL	0	NULL	Migrants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Migrants traveling to their country of origin : a bridge population for HIV transmission ?
	manualset3
218235	2	420234	7	NULL	NULL	0	NULL	country of origin	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Migrants traveling to their country of origin : a bridge population for HIV transmission ?
	manualset3
218236	3	420234	7	NULL	NULL	0	NULL	bridge population 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Migrants traveling to their country of origin : a bridge population for HIV transmission ?
	manualset3
218237	4	420234	7	NULL	NULL	NULL	NULL	HIV transmission 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Migrants traveling to their country of origin : a bridge population for HIV transmission ?
	manualset3
218238	1	420235	7	NULL	NULL	0	NULL	Conversion 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Conversion of 4-nitroquinoline 1-oxide to 4-aminoquinoline 1-oxide by rat liver enzymes .
	manualset3
218239	2	420235	7	NULL	NULL	0	NULL	4-nitroquinoline 1-oxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Conversion of 4-nitroquinoline 1-oxide to 4-aminoquinoline 1-oxide by rat liver enzymes .
	manualset3
218240	3	420235	7	NULL	NULL	0	NULL	4-aminoquinoline 1-oxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Conversion of 4-nitroquinoline 1-oxide to 4-aminoquinoline 1-oxide by rat liver enzymes .
	manualset3
218241	4	420235	7	NULL	NULL	0	NULL	rat liver enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Conversion of 4-nitroquinoline 1-oxide to 4-aminoquinoline 1-oxide by rat liver enzymes .
	manualset3
218242	1	420236	7	NULL	NULL	0	NULL	regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of blood flow is achieved by the combined effects of multiple interacting mechanisms , including sensitivity to pressure , flow rate , metabolite levels , and neural signals .
	manualset3
218243	2	420236	7	NULL	NULL	0	NULL	blood flow	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of blood flow is achieved by the combined effects of multiple interacting mechanisms , including sensitivity to pressure , flow rate , metabolite levels , and neural signals .
	manualset3
218244	3	420236	7	NULL	NULL	0	NULL	combined effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of blood flow is achieved by the combined effects of multiple interacting mechanisms , including sensitivity to pressure , flow rate , metabolite levels , and neural signals .
	manualset3
218245	4	420236	7	NULL	NULL	0	NULL	multiple interacting mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of blood flow is achieved by the combined effects of multiple interacting mechanisms , including sensitivity to pressure , flow rate , metabolite levels , and neural signals .
	manualset3
218246	5	420236	7	NULL	NULL	0	NULL	sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of blood flow is achieved by the combined effects of multiple interacting mechanisms , including sensitivity to pressure , flow rate , metabolite levels , and neural signals .
	manualset3
218247	6	420236	7	NULL	NULL	0	NULL	Pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of blood flow is achieved by the combined effects of multiple interacting mechanisms , including sensitivity to pressure , flow rate , metabolite levels , and neural signals .
	manualset3
219837	7	420236	7	NULL	NULL	0	NULL	flow rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of blood flow is achieved by the combined effects of multiple interacting mechanisms , including sensitivity to pressure , flow rate , metabolite levels , and neural signals .
	manualset3
219838	8	420236	7	NULL	NULL	0	NULL	metabolite levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of blood flow is achieved by the combined effects of multiple interacting mechanisms , including sensitivity to pressure , flow rate , metabolite levels , and neural signals .
	manualset3
219839	9	420236	7	NULL	NULL	0	NULL	neural signals	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of blood flow is achieved by the combined effects of multiple interacting mechanisms , including sensitivity to pressure , flow rate , metabolite levels , and neural signals .
	manualset3
218248	1	420237	7	NULL	NULL	0	NULL	Implications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Implications for development and management of telemedicine also are discussed .
	manualset3
218249	2	420237	7	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Implications for development and management of telemedicine also are discussed .
	manualset3
218250	3	420237	7	NULL	NULL	0	NULL	management 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Implications for development and management of telemedicine also are discussed .
	manualset3
218251	4	420237	7	NULL	NULL	0	NULL	 telemedicine	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Implications for development and management of telemedicine also are discussed .
	manualset3
218252	1	420238	7	NULL	NULL	0	NULL	Gabriel Boughton	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Gabriel Boughton and William Hamilton : surgeons who helped build British power in India .
	manualset3
218253	2	420238	7	NULL	NULL	0	NULL	William Hamilton	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Gabriel Boughton and William Hamilton : surgeons who helped build British power in India .
	manualset3
218254	3	420238	7	NULL	NULL	0	NULL	 surgeons	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Gabriel Boughton and William Hamilton : surgeons who helped build British power in India .
	manualset3
218255	4	420238	7	NULL	NULL	0	NULL	British power 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Gabriel Boughton and William Hamilton : surgeons who helped build British power in India .
	manualset3
218256	5	420238	7	NULL	NULL	0	NULL	India 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Gabriel Boughton and William Hamilton : surgeons who helped build British power in India .
	manualset3
218257	1	420239	7	NULL	NULL	0	NULL	no overt differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there were no overt differences in embryo viability between cryoprotectant treatments ( each resulted in live offspring after embryo transfer ) , there was a lower ( P & lt ; 0.01 ) incidence of zona pellucida damage using propylene glycol ( 4 % ) compared to glycerol ( 40 % ) .
	manualset3
218258	2	420239	7	NULL	NULL	0	NULL	embryo viability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there were no overt differences in embryo viability between cryoprotectant treatments ( each resulted in live offspring after embryo transfer ) , there was a lower ( P & lt ; 0.01 ) incidence of zona pellucida damage using propylene glycol ( 4 % ) compared to glycerol ( 40 % ) .
	manualset3
218259	3	420239	7	NULL	NULL	0	NULL	cryoprotectant treatments 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there were no overt differences in embryo viability between cryoprotectant treatments ( each resulted in live offspring after embryo transfer ) , there was a lower ( P & lt ; 0.01 ) incidence of zona pellucida damage using propylene glycol ( 4 % ) compared to glycerol ( 40 % ) .
	manualset3
218260	4	420239	7	NULL	NULL	0	NULL	 live offspring	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there were no overt differences in embryo viability between cryoprotectant treatments ( each resulted in live offspring after embryo transfer ) , there was a lower ( P & lt ; 0.01 ) incidence of zona pellucida damage using propylene glycol ( 4 % ) compared to glycerol ( 40 % ) .
	manualset3
218261	5	420239	7	NULL	NULL	0	NULL	embryo transfer	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there were no overt differences in embryo viability between cryoprotectant treatments ( each resulted in live offspring after embryo transfer ) , there was a lower ( P & lt ; 0.01 ) incidence of zona pellucida damage using propylene glycol ( 4 % ) compared to glycerol ( 40 % ) .
	manualset3
218262	6	420239	7	NULL	NULL	0	NULL	 P & lt ; 0.01	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there were no overt differences in embryo viability between cryoprotectant treatments ( each resulted in live offspring after embryo transfer ) , there was a lower ( P & lt ; 0.01 ) incidence of zona pellucida damage using propylene glycol ( 4 % ) compared to glycerol ( 40 % ) .
	manualset3
218263	7	420239	7	NULL	NULL	0	NULL	incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there were no overt differences in embryo viability between cryoprotectant treatments ( each resulted in live offspring after embryo transfer ) , there was a lower ( P & lt ; 0.01 ) incidence of zona pellucida damage using propylene glycol ( 4 % ) compared to glycerol ( 40 % ) .
	manualset3
218264	8	420239	7	NULL	NULL	0	NULL	zona pellucida damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there were no overt differences in embryo viability between cryoprotectant treatments ( each resulted in live offspring after embryo transfer ) , there was a lower ( P & lt ; 0.01 ) incidence of zona pellucida damage using propylene glycol ( 4 % ) compared to glycerol ( 40 % ) .
	manualset3
218265	9	420239	7	NULL	NULL	0	NULL	propylene glycol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there were no overt differences in embryo viability between cryoprotectant treatments ( each resulted in live offspring after embryo transfer ) , there was a lower ( P & lt ; 0.01 ) incidence of zona pellucida damage using propylene glycol ( 4 % ) compared to glycerol ( 40 % ) .
	manualset3
218267	11	420239	7	NULL	NULL	0	NULL	4 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there were no overt differences in embryo viability between cryoprotectant treatments ( each resulted in live offspring after embryo transfer ) , there was a lower ( P & lt ; 0.01 ) incidence of zona pellucida damage using propylene glycol ( 4 % ) compared to glycerol ( 40 % ) .
	manualset3
218268	12	420239	7	NULL	NULL	0	NULL	glycerol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there were no overt differences in embryo viability between cryoprotectant treatments ( each resulted in live offspring after embryo transfer ) , there was a lower ( P & lt ; 0.01 ) incidence of zona pellucida damage using propylene glycol ( 4 % ) compared to glycerol ( 40 % ) .
	manualset3
218269	13	420239	7	NULL	NULL	0	NULL	40 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there were no overt differences in embryo viability between cryoprotectant treatments ( each resulted in live offspring after embryo transfer ) , there was a lower ( P & lt ; 0.01 ) incidence of zona pellucida damage using propylene glycol ( 4 % ) compared to glycerol ( 40 % ) .
	manualset3
218270	1	420240	7	NULL	NULL	0	NULL	carboxyl-terminal regions	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thereafter , carboxyl-terminal regions of the fibrin a-chains are thought to be untethered and interact with those of other protofibrils leading to the formation of thick fibrin bundles and interwoven networks after appropriate branching ( 6-9 ) .
	manualset3
218271	2	420240	7	NULL	NULL	0	NULL	fibrin a-chains 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thereafter , carboxyl-terminal regions of the fibrin a-chains are thought to be untethered and interact with those of other protofibrils leading to the formation of thick fibrin bundles and interwoven networks after appropriate branching ( 6-9 ) .
	manualset3
218272	3	420240	7	NULL	NULL	0	NULL	protofibrils	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thereafter , carboxyl-terminal regions of the fibrin a-chains are thought to be untethered and interact with those of other protofibrils leading to the formation of thick fibrin bundles and interwoven networks after appropriate branching ( 6-9 ) .
	manualset3
218273	4	420240	7	NULL	NULL	0	NULL	formation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Thereafter , carboxyl-terminal regions of the fibrin a-chains are thought to be untethered and interact with those of other protofibrils leading to the formation of thick fibrin bundles and interwoven networks after appropriate branching ( 6-9 ) .
	manualset3
218274	5	420240	7	NULL	NULL	0	NULL	thick fibrin bundles	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thereafter , carboxyl-terminal regions of the fibrin a-chains are thought to be untethered and interact with those of other protofibrils leading to the formation of thick fibrin bundles and interwoven networks after appropriate branching ( 6-9 ) .
	manualset3
218275	6	420240	7	NULL	NULL	0	NULL	interwoven networks	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thereafter , carboxyl-terminal regions of the fibrin a-chains are thought to be untethered and interact with those of other protofibrils leading to the formation of thick fibrin bundles and interwoven networks after appropriate branching ( 6-9 ) .
	manualset3
218276	7	420240	7	NULL	NULL	0	NULL	branching ( 6-9 )	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thereafter , carboxyl-terminal regions of the fibrin a-chains are thought to be untethered and interact with those of other protofibrils leading to the formation of thick fibrin bundles and interwoven networks after appropriate branching ( 6-9 ) .
	manualset3
218277	1	420241	7	NULL	NULL	0	NULL	Proceedings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Proceedings : Adaptation of synaptic transmission between hair-cells and the 8th nerve ) .
	manualset3
218278	2	420241	7	NULL	NULL	0	NULL	Adaptation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Proceedings : Adaptation of synaptic transmission between hair-cells and the 8th nerve ) .
	manualset3
218279	3	420241	7	NULL	NULL	0	NULL	synaptic transmission	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Proceedings : Adaptation of synaptic transmission between hair-cells and the 8th nerve ) .
	manualset3
218280	4	420241	7	NULL	NULL	0	NULL	hair-cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	( Proceedings : Adaptation of synaptic transmission between hair-cells and the 8th nerve ) .
	manualset3
218281	5	420241	7	NULL	NULL	0	NULL	8th nerve 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Proceedings : Adaptation of synaptic transmission between hair-cells and the 8th nerve ) .
	manualset3
218282	1	420242	7	NULL	NULL	0	NULL	Results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results were related to HbA ( 1c ) and were compared to those of 97 healthy controls .
	manualset3
218283	2	420242	7	NULL	NULL	0	NULL	HbA ( 1c )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Results were related to HbA ( 1c ) and were compared to those of 97 healthy controls .
	manualset3
218284	3	420242	7	NULL	NULL	0	NULL	97 healthy controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Results were related to HbA ( 1c ) and were compared to those of 97 healthy controls .
	manualset3
218285	1	420243	7	NULL	NULL	0	NULL	total 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 385 adult flukes collected from 10 patients were morphologically identified to species and defined as Clonorchis sinensis ( 14.58 % ) in Opisthorchiidae family , Haplorchis taichui ( 32.29 % ) , Haplorchis pumilio ( 52.08 % ) and Centrocestus formosanus ( 1.04 % ) in Heterophyidae family .
	manualset3
218286	2	420243	7	NULL	NULL	0	NULL	385 adult flukes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 385 adult flukes collected from 10 patients were morphologically identified to species and defined as Clonorchis sinensis ( 14.58 % ) in Opisthorchiidae family , Haplorchis taichui ( 32.29 % ) , Haplorchis pumilio ( 52.08 % ) and Centrocestus formosanus ( 1.04 % ) in Heterophyidae family .
	manualset3
218287	3	420243	7	NULL	NULL	0	NULL	10 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 385 adult flukes collected from 10 patients were morphologically identified to species and defined as Clonorchis sinensis ( 14.58 % ) in Opisthorchiidae family , Haplorchis taichui ( 32.29 % ) , Haplorchis pumilio ( 52.08 % ) and Centrocestus formosanus ( 1.04 % ) in Heterophyidae family .
	manualset3
218288	4	420243	7	NULL	NULL	0	NULL	species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 385 adult flukes collected from 10 patients were morphologically identified to species and defined as Clonorchis sinensis ( 14.58 % ) in Opisthorchiidae family , Haplorchis taichui ( 32.29 % ) , Haplorchis pumilio ( 52.08 % ) and Centrocestus formosanus ( 1.04 % ) in Heterophyidae family .
	manualset3
218289	5	420243	7	NULL	NULL	0	NULL	Clonorchis sinensis 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 385 adult flukes collected from 10 patients were morphologically identified to species and defined as Clonorchis sinensis ( 14.58 % ) in Opisthorchiidae family , Haplorchis taichui ( 32.29 % ) , Haplorchis pumilio ( 52.08 % ) and Centrocestus formosanus ( 1.04 % ) in Heterophyidae family .
	manualset3
218290	6	420243	7	NULL	NULL	0	NULL	14.58 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 385 adult flukes collected from 10 patients were morphologically identified to species and defined as Clonorchis sinensis ( 14.58 % ) in Opisthorchiidae family , Haplorchis taichui ( 32.29 % ) , Haplorchis pumilio ( 52.08 % ) and Centrocestus formosanus ( 1.04 % ) in Heterophyidae family .
	manualset3
218291	7	420243	7	NULL	NULL	0	NULL	Opisthorchiidae family	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 385 adult flukes collected from 10 patients were morphologically identified to species and defined as Clonorchis sinensis ( 14.58 % ) in Opisthorchiidae family , Haplorchis taichui ( 32.29 % ) , Haplorchis pumilio ( 52.08 % ) and Centrocestus formosanus ( 1.04 % ) in Heterophyidae family .
	manualset3
218292	8	420243	7	NULL	NULL	0	NULL	Haplorchis taichui 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 385 adult flukes collected from 10 patients were morphologically identified to species and defined as Clonorchis sinensis ( 14.58 % ) in Opisthorchiidae family , Haplorchis taichui ( 32.29 % ) , Haplorchis pumilio ( 52.08 % ) and Centrocestus formosanus ( 1.04 % ) in Heterophyidae family .
	manualset3
218293	9	420243	7	NULL	NULL	0	NULL	32.29 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 385 adult flukes collected from 10 patients were morphologically identified to species and defined as Clonorchis sinensis ( 14.58 % ) in Opisthorchiidae family , Haplorchis taichui ( 32.29 % ) , Haplorchis pumilio ( 52.08 % ) and Centrocestus formosanus ( 1.04 % ) in Heterophyidae family .
	manualset3
218294	10	420243	7	NULL	NULL	0	NULL	Haplorchis pumilio	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 385 adult flukes collected from 10 patients were morphologically identified to species and defined as Clonorchis sinensis ( 14.58 % ) in Opisthorchiidae family , Haplorchis taichui ( 32.29 % ) , Haplorchis pumilio ( 52.08 % ) and Centrocestus formosanus ( 1.04 % ) in Heterophyidae family .
	manualset3
218295	11	420243	7	NULL	NULL	0	NULL	52.08 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 385 adult flukes collected from 10 patients were morphologically identified to species and defined as Clonorchis sinensis ( 14.58 % ) in Opisthorchiidae family , Haplorchis taichui ( 32.29 % ) , Haplorchis pumilio ( 52.08 % ) and Centrocestus formosanus ( 1.04 % ) in Heterophyidae family .
	manualset3
218296	12	420243	7	NULL	NULL	0	NULL	Centrocestus formosanus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 385 adult flukes collected from 10 patients were morphologically identified to species and defined as Clonorchis sinensis ( 14.58 % ) in Opisthorchiidae family , Haplorchis taichui ( 32.29 % ) , Haplorchis pumilio ( 52.08 % ) and Centrocestus formosanus ( 1.04 % ) in Heterophyidae family .
	manualset3
218297	13	420243	7	NULL	NULL	0	NULL	1.04 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 385 adult flukes collected from 10 patients were morphologically identified to species and defined as Clonorchis sinensis ( 14.58 % ) in Opisthorchiidae family , Haplorchis taichui ( 32.29 % ) , Haplorchis pumilio ( 52.08 % ) and Centrocestus formosanus ( 1.04 % ) in Heterophyidae family .
	manualset3
218298	14	420243	7	NULL	NULL	0	NULL	Heterophyidae family 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A total of 385 adult flukes collected from 10 patients were morphologically identified to species and defined as Clonorchis sinensis ( 14.58 % ) in Opisthorchiidae family , Haplorchis taichui ( 32.29 % ) , Haplorchis pumilio ( 52.08 % ) and Centrocestus formosanus ( 1.04 % ) in Heterophyidae family .
	manualset3
218299	1	420244	7	NULL	NULL	0	NULL	1 horse	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Only 1 horse had epiglottic entrapment .
	manualset3
218300	2	420244	7	NULL	NULL	0	NULL	epiglottic entrapment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Only 1 horse had epiglottic entrapment .
	manualset3
218301	1	420245	7	NULL	NULL	0	NULL	 information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	To obtain information about the propulsion caused by the leg , we made elongated and stiff cells using a detergent .
	manualset3
218302	2	420245	7	NULL	NULL	0	NULL	propulsion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To obtain information about the propulsion caused by the leg , we made elongated and stiff cells using a detergent .
	manualset3
218303	3	420245	7	NULL	NULL	0	NULL	leg	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To obtain information about the propulsion caused by the leg , we made elongated and stiff cells using a detergent .
	manualset3
218304	4	420245	7	NULL	NULL	0	NULL	stiff cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To obtain information about the propulsion caused by the leg , we made elongated and stiff cells using a detergent .
	manualset3
218305	5	420245	7	NULL	NULL	0	NULL	detergent 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To obtain information about the propulsion caused by the leg , we made elongated and stiff cells using a detergent .
	manualset3
218306	1	420246	7	NULL	NULL	0	NULL	smallest CBP	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The smallest CBP occur as monomeric peptides with a molecular weight of approximately 8.5 kDa .
	manualset3
218307	2	420246	7	NULL	NULL	0	NULL	monomeric peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The smallest CBP occur as monomeric peptides with a molecular weight of approximately 8.5 kDa .
	manualset3
218308	3	420246	7	NULL	NULL	0	NULL	molecular weight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The smallest CBP occur as monomeric peptides with a molecular weight of approximately 8.5 kDa .
	manualset3
218309	4	420246	7	NULL	NULL	0	NULL	 8.5 kDa 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The smallest CBP occur as monomeric peptides with a molecular weight of approximately 8.5 kDa .
	manualset3
218310	1	420247	7	NULL	NULL	0	NULL	average child death rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average child death rate due to electrocution was 1.42 per 100 , 000 population-year .
	manualset3
218311	2	420247	7	NULL	NULL	0	NULL	electrocution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The average child death rate due to electrocution was 1.42 per 100 , 000 population-year .
	manualset3
218312	3	420247	7	NULL	NULL	0	NULL	1.42 per 100 , 000 population-year	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average child death rate due to electrocution was 1.42 per 100 , 000 population-year .
	manualset3
218313	1	420248	7	NULL	NULL	0	NULL	Efficacy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Efficacy of a novel formulation of metaflumizone plus amitraz for the treatment of sarcoptic mange in dogs .
	manualset3
218314	2	420248	7	NULL	NULL	NULL	NULL	novel formulation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Efficacy of a novel formulation of metaflumizone plus amitraz for the treatment of sarcoptic mange in dogs .
	manualset3
218315	3	420248	7	NULL	NULL	0	NULL	metaflumizone plus amitraz	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Efficacy of a novel formulation of metaflumizone plus amitraz for the treatment of sarcoptic mange in dogs .
	manualset3
218316	4	420248	7	NULL	NULL	0	NULL	 treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Efficacy of a novel formulation of metaflumizone plus amitraz for the treatment of sarcoptic mange in dogs .
	manualset3
218317	5	420248	7	NULL	NULL	0	NULL	sarcoptic mange	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Efficacy of a novel formulation of metaflumizone plus amitraz for the treatment of sarcoptic mange in dogs .
	manualset3
218318	6	420248	7	NULL	NULL	0	NULL	dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Efficacy of a novel formulation of metaflumizone plus amitraz for the treatment of sarcoptic mange in dogs .
	manualset3
218319	1	420249	7	NULL	NULL	0	NULL	Evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence suggests that extinction , the suppression of a learned response to a Pavlovian signal that is produced by exposure to the signal alone after conditioning , is a consequence of new inhibitory learning .
	manualset3
218320	2	420249	7	NULL	NULL	0	NULL	extinction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence suggests that extinction , the suppression of a learned response to a Pavlovian signal that is produced by exposure to the signal alone after conditioning , is a consequence of new inhibitory learning .
	manualset3
218321	3	420249	7	NULL	NULL	NULL	NULL	suppression	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Evidence suggests that extinction , the suppression of a learned response to a Pavlovian signal that is produced by exposure to the signal alone after conditioning , is a consequence of new inhibitory learning .
	manualset3
218322	4	420249	7	NULL	NULL	0	NULL	learned response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence suggests that extinction , the suppression of a learned response to a Pavlovian signal that is produced by exposure to the signal alone after conditioning , is a consequence of new inhibitory learning .
	manualset3
218323	5	420249	7	NULL	NULL	0	NULL	Pavlovian signal 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence suggests that extinction , the suppression of a learned response to a Pavlovian signal that is produced by exposure to the signal alone after conditioning , is a consequence of new inhibitory learning .
	manualset3
218324	6	420249	7	NULL	NULL	0	NULL	 signal	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence suggests that extinction , the suppression of a learned response to a Pavlovian signal that is produced by exposure to the signal alone after conditioning , is a consequence of new inhibitory learning .
	manualset3
218325	8	420249	7	NULL	NULL	NULL	NULL	 new inhibitory learning	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Evidence suggests that extinction , the suppression of a learned response to a Pavlovian signal that is produced by exposure to the signal alone after conditioning , is a consequence of new inhibitory learning .
	manualset3
218326	7	420249	7	NULL	NULL	NULL	NULL	conditioning	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Evidence suggests that extinction , the suppression of a learned response to a Pavlovian signal that is produced by exposure to the signal alone after conditioning , is a consequence of new inhibitory learning .
	manualset3
218327	1	420250	7	NULL	NULL	0	NULL	1982	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1982 , the policy indicated that abortion could be induced if the pregnant woman is over 35 .
	manualset3
218328	2	420250	7	NULL	NULL	0	NULL	policy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1982 , the policy indicated that abortion could be induced if the pregnant woman is over 35 .
	manualset3
218329	3	420250	7	NULL	NULL	0	NULL	abortion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1982 , the policy indicated that abortion could be induced if the pregnant woman is over 35 .
	manualset3
218330	4	420250	7	NULL	NULL	0	NULL	pregnant woman	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1982 , the policy indicated that abortion could be induced if the pregnant woman is over 35 .
	manualset3
218331	5	420250	7	NULL	NULL	0	NULL	35	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1982 , the policy indicated that abortion could be induced if the pregnant woman is over 35 .
	manualset3
218332	1	420251	7	NULL	NULL	0	NULL	V1-receptor antagonist ( 1 - ( beta-mercapto-beta , beta-cyclopentamethylene proprionic acid )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The V1-receptor antagonist ( 1 - ( beta-mercapto-beta , beta-cyclopentamethylene proprionic acid ) , 2 - ( O-methyl-Tyr ) - Arg ) vasopressin ( PMP ) inhibited only AVP-induced promotion of MC growth ( maximal inhibition of -78.3 % ) .
	manualset3
218333	2	420251	7	NULL	NULL	0	NULL	2 - ( O-methyl-Tyr ) - Arg ) vasopressin ( PMP )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The V1-receptor antagonist ( 1 - ( beta-mercapto-beta , beta-cyclopentamethylene proprionic acid ) , 2 - ( O-methyl-Tyr ) - Arg ) vasopressin ( PMP ) inhibited only AVP-induced promotion of MC growth ( maximal inhibition of -78.3 % ) .
	manualset3
218334	3	420251	7	NULL	NULL	NULL	NULL	AVP-induced promotion 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The V1-receptor antagonist ( 1 - ( beta-mercapto-beta , beta-cyclopentamethylene proprionic acid ) , 2 - ( O-methyl-Tyr ) - Arg ) vasopressin ( PMP ) inhibited only AVP-induced promotion of MC growth ( maximal inhibition of -78.3 % ) .
	manualset3
218335	4	420251	7	NULL	NULL	0	NULL	MC growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The V1-receptor antagonist ( 1 - ( beta-mercapto-beta , beta-cyclopentamethylene proprionic acid ) , 2 - ( O-methyl-Tyr ) - Arg ) vasopressin ( PMP ) inhibited only AVP-induced promotion of MC growth ( maximal inhibition of -78.3 % ) .
	manualset3
218336	5	420251	7	NULL	NULL	0	NULL	maximal inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The V1-receptor antagonist ( 1 - ( beta-mercapto-beta , beta-cyclopentamethylene proprionic acid ) , 2 - ( O-methyl-Tyr ) - Arg ) vasopressin ( PMP ) inhibited only AVP-induced promotion of MC growth ( maximal inhibition of -78.3 % ) .
	manualset3
218337	6	420251	7	NULL	NULL	0	NULL	-78.3 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The V1-receptor antagonist ( 1 - ( beta-mercapto-beta , beta-cyclopentamethylene proprionic acid ) , 2 - ( O-methyl-Tyr ) - Arg ) vasopressin ( PMP ) inhibited only AVP-induced promotion of MC growth ( maximal inhibition of -78.3 % ) .
	manualset3
218338	1	420252	7	NULL	NULL	0	NULL	 dissociation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For the dissociation of HF dimers , the anharmonic rate constants are around 3.02 x 10 ( 10 ) to 3.46 x 10 ( 12 ) s ( -1 ) , while the harmonic rate constants are in the range of 2.93 x 10 ( 10 ) to 1.66 x 10 ( 13 ) s ( -1 ) , at a temperature range of 243-1000 K , for the canonical case .
	manualset3
218339	2	420252	7	NULL	NULL	0	NULL	HF dimers	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	For the dissociation of HF dimers , the anharmonic rate constants are around 3.02 x 10 ( 10 ) to 3.46 x 10 ( 12 ) s ( -1 ) , while the harmonic rate constants are in the range of 2.93 x 10 ( 10 ) to 1.66 x 10 ( 13 ) s ( -1 ) , at a temperature range of 243-1000 K , for the canonical case .
	manualset3
218340	3	420252	7	NULL	NULL	0	NULL	anharmonic rate constants	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the dissociation of HF dimers , the anharmonic rate constants are around 3.02 x 10 ( 10 ) to 3.46 x 10 ( 12 ) s ( -1 ) , while the harmonic rate constants are in the range of 2.93 x 10 ( 10 ) to 1.66 x 10 ( 13 ) s ( -1 ) , at a temperature range of 243-1000 K , for the canonical case .
	manualset3
218341	4	420252	7	NULL	NULL	0	NULL	3.02 x 10 ( 10 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the dissociation of HF dimers , the anharmonic rate constants are around 3.02 x 10 ( 10 ) to 3.46 x 10 ( 12 ) s ( -1 ) , while the harmonic rate constants are in the range of 2.93 x 10 ( 10 ) to 1.66 x 10 ( 13 ) s ( -1 ) , at a temperature range of 243-1000 K , for the canonical case .
	manualset3
218342	5	420252	7	NULL	NULL	0	NULL	3.46 x 10 ( 12 ) s ( -1 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the dissociation of HF dimers , the anharmonic rate constants are around 3.02 x 10 ( 10 ) to 3.46 x 10 ( 12 ) s ( -1 ) , while the harmonic rate constants are in the range of 2.93 x 10 ( 10 ) to 1.66 x 10 ( 13 ) s ( -1 ) , at a temperature range of 243-1000 K , for the canonical case .
	manualset3
218343	6	420252	7	NULL	NULL	0	NULL	harmonic rate constants	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the dissociation of HF dimers , the anharmonic rate constants are around 3.02 x 10 ( 10 ) to 3.46 x 10 ( 12 ) s ( -1 ) , while the harmonic rate constants are in the range of 2.93 x 10 ( 10 ) to 1.66 x 10 ( 13 ) s ( -1 ) , at a temperature range of 243-1000 K , for the canonical case .
	manualset3
218344	7	420252	7	NULL	NULL	0	NULL	 range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the dissociation of HF dimers , the anharmonic rate constants are around 3.02 x 10 ( 10 ) to 3.46 x 10 ( 12 ) s ( -1 ) , while the harmonic rate constants are in the range of 2.93 x 10 ( 10 ) to 1.66 x 10 ( 13 ) s ( -1 ) , at a temperature range of 243-1000 K , for the canonical case .
	manualset3
218345	8	420252	7	NULL	NULL	0	NULL	2.93 x 10 ( 10 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the dissociation of HF dimers , the anharmonic rate constants are around 3.02 x 10 ( 10 ) to 3.46 x 10 ( 12 ) s ( -1 ) , while the harmonic rate constants are in the range of 2.93 x 10 ( 10 ) to 1.66 x 10 ( 13 ) s ( -1 ) , at a temperature range of 243-1000 K , for the canonical case .
	manualset3
218346	9	420252	7	NULL	NULL	0	NULL	1.66 x 10 ( 13 ) s ( -1 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the dissociation of HF dimers , the anharmonic rate constants are around 3.02 x 10 ( 10 ) to 3.46 x 10 ( 12 ) s ( -1 ) , while the harmonic rate constants are in the range of 2.93 x 10 ( 10 ) to 1.66 x 10 ( 13 ) s ( -1 ) , at a temperature range of 243-1000 K , for the canonical case .
	manualset3
218347	10	420252	7	NULL	NULL	0	NULL	temperature range	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For the dissociation of HF dimers , the anharmonic rate constants are around 3.02 x 10 ( 10 ) to 3.46 x 10 ( 12 ) s ( -1 ) , while the harmonic rate constants are in the range of 2.93 x 10 ( 10 ) to 1.66 x 10 ( 13 ) s ( -1 ) , at a temperature range of 243-1000 K , for the canonical case .
	manualset3
218348	11	420252	7	NULL	NULL	0	NULL	243-1000 K	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the dissociation of HF dimers , the anharmonic rate constants are around 3.02 x 10 ( 10 ) to 3.46 x 10 ( 12 ) s ( -1 ) , while the harmonic rate constants are in the range of 2.93 x 10 ( 10 ) to 1.66 x 10 ( 13 ) s ( -1 ) , at a temperature range of 243-1000 K , for the canonical case .
	manualset3
218349	12	420252	7	NULL	NULL	0	NULL	canonical case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For the dissociation of HF dimers , the anharmonic rate constants are around 3.02 x 10 ( 10 ) to 3.46 x 10 ( 12 ) s ( -1 ) , while the harmonic rate constants are in the range of 2.93 x 10 ( 10 ) to 1.66 x 10 ( 13 ) s ( -1 ) , at a temperature range of 243-1000 K , for the canonical case .
	manualset3
218350	1	420253	7	NULL	NULL	0	NULL	growth rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these growth rates varied from 3.80 to 9.50 g/days and large variations in growth rate were observed between litters , the findings suggest that development within a pouch , in contrast to uterine development , gives rise to a litter which is more uniform in size .
	manualset3
218351	2	420253	7	NULL	NULL	NULL	NULL	3.80 g/days	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although these growth rates varied from 3.80 to 9.50 g/days and large variations in growth rate were observed between litters , the findings suggest that development within a pouch , in contrast to uterine development , gives rise to a litter which is more uniform in size .
	manualset3
218352	3	420253	7	NULL	NULL	0	NULL	9.50 g/days	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these growth rates varied from 3.80 to 9.50 g/days and large variations in growth rate were observed between litters , the findings suggest that development within a pouch , in contrast to uterine development , gives rise to a litter which is more uniform in size .
	manualset3
218353	4	420253	7	NULL	NULL	0	NULL	large variations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these growth rates varied from 3.80 to 9.50 g/days and large variations in growth rate were observed between litters , the findings suggest that development within a pouch , in contrast to uterine development , gives rise to a litter which is more uniform in size .
	manualset3
218354	5	420253	7	NULL	NULL	0	NULL	growth rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these growth rates varied from 3.80 to 9.50 g/days and large variations in growth rate were observed between litters , the findings suggest that development within a pouch , in contrast to uterine development , gives rise to a litter which is more uniform in size .
	manualset3
218355	6	420253	7	NULL	NULL	0	NULL	litters	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these growth rates varied from 3.80 to 9.50 g/days and large variations in growth rate were observed between litters , the findings suggest that development within a pouch , in contrast to uterine development , gives rise to a litter which is more uniform in size .
	manualset3
218356	7	420253	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these growth rates varied from 3.80 to 9.50 g/days and large variations in growth rate were observed between litters , the findings suggest that development within a pouch , in contrast to uterine development , gives rise to a litter which is more uniform in size .
	manualset3
218357	8	420253	7	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these growth rates varied from 3.80 to 9.50 g/days and large variations in growth rate were observed between litters , the findings suggest that development within a pouch , in contrast to uterine development , gives rise to a litter which is more uniform in size .
	manualset3
218358	9	420253	7	NULL	NULL	0	NULL	pouch	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these growth rates varied from 3.80 to 9.50 g/days and large variations in growth rate were observed between litters , the findings suggest that development within a pouch , in contrast to uterine development , gives rise to a litter which is more uniform in size .
	manualset3
218359	10	420253	7	NULL	NULL	0	NULL	uterine development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these growth rates varied from 3.80 to 9.50 g/days and large variations in growth rate were observed between litters , the findings suggest that development within a pouch , in contrast to uterine development , gives rise to a litter which is more uniform in size .
	manualset3
218360	11	420253	7	NULL	NULL	0	NULL	litter	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these growth rates varied from 3.80 to 9.50 g/days and large variations in growth rate were observed between litters , the findings suggest that development within a pouch , in contrast to uterine development , gives rise to a litter which is more uniform in size .
	manualset3
218361	12	420253	7	NULL	NULL	0	NULL	size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these growth rates varied from 3.80 to 9.50 g/days and large variations in growth rate were observed between litters , the findings suggest that development within a pouch , in contrast to uterine development , gives rise to a litter which is more uniform in size .
	manualset3
218362	1	420254	7	NULL	NULL	0	NULL	treated rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The treated rats developed with a distinct facial appearance characterized by a markedly reduced snout .
	manualset3
218363	2	420254	7	NULL	NULL	0	NULL	facial appearance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The treated rats developed with a distinct facial appearance characterized by a markedly reduced snout .
	manualset3
218364	3	420254	7	NULL	NULL	0	NULL	markedly reduced snout 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The treated rats developed with a distinct facial appearance characterized by a markedly reduced snout .
	manualset3
218365	1	420255	7	NULL	NULL	0	NULL	condition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The condition is often confused with other surgical emergencies such as appendicitis and ectopic pregnancy .
	manualset3
218366	2	420255	7	NULL	NULL	0	NULL	surgical emergencies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The condition is often confused with other surgical emergencies such as appendicitis and ectopic pregnancy .
	manualset3
218367	3	420255	7	NULL	NULL	0	NULL	appendicitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The condition is often confused with other surgical emergencies such as appendicitis and ectopic pregnancy .
	manualset3
218368	4	420255	7	NULL	NULL	0	NULL	ectopic pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The condition is often confused with other surgical emergencies such as appendicitis and ectopic pregnancy .
	manualset3
218369	1	420256	7	NULL	NULL	0	NULL	Aggravation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Aggravation by morphine and D-aspartic acid of pyelonephritis induced by i.v. inoculation of Staphylococcus aureus in rats .
	manualset3
218370	2	420256	7	NULL	NULL	0	NULL	morphine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Aggravation by morphine and D-aspartic acid of pyelonephritis induced by i.v. inoculation of Staphylococcus aureus in rats .
	manualset3
218371	3	420256	7	NULL	NULL	0	NULL	D-aspartic acid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Aggravation by morphine and D-aspartic acid of pyelonephritis induced by i.v. inoculation of Staphylococcus aureus in rats .
	manualset3
218372	4	420256	7	NULL	NULL	0	NULL	 pyelonephritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Aggravation by morphine and D-aspartic acid of pyelonephritis induced by i.v. inoculation of Staphylococcus aureus in rats .
	manualset3
218373	5	420256	7	NULL	NULL	0	NULL	i.v. inoculation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Aggravation by morphine and D-aspartic acid of pyelonephritis induced by i.v. inoculation of Staphylococcus aureus in rats .
	manualset3
218374	6	420256	7	NULL	NULL	0	NULL	Staphylococcus aureus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Aggravation by morphine and D-aspartic acid of pyelonephritis induced by i.v. inoculation of Staphylococcus aureus in rats .
	manualset3
218375	7	420256	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Aggravation by morphine and D-aspartic acid of pyelonephritis induced by i.v. inoculation of Staphylococcus aureus in rats .
	manualset3
218376	1	420257	7	NULL	NULL	0	NULL	mRNA level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidentally , mRNA level of caveolin-3 and peroxisome proliferator activated receptor gamma coactivator-1alpha was also significantly decreased 14 d after myostatin gene electrotransfer .
	manualset3
218377	2	420257	7	NULL	NULL	0	NULL	caveolin-3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidentally , mRNA level of caveolin-3 and peroxisome proliferator activated receptor gamma coactivator-1alpha was also significantly decreased 14 d after myostatin gene electrotransfer .
	manualset3
218378	3	420257	7	NULL	NULL	0	NULL	peroxisome proliferator activated receptor gamma coactivator-1alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidentally , mRNA level of caveolin-3 and peroxisome proliferator activated receptor gamma coactivator-1alpha was also significantly decreased 14 d after myostatin gene electrotransfer .
	manualset3
218379	4	420257	7	NULL	NULL	0	NULL	14 d	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidentally , mRNA level of caveolin-3 and peroxisome proliferator activated receptor gamma coactivator-1alpha was also significantly decreased 14 d after myostatin gene electrotransfer .
	manualset3
218380	5	420257	7	NULL	NULL	0	NULL	myostatin gene electrotransfer	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Incidentally , mRNA level of caveolin-3 and peroxisome proliferator activated receptor gamma coactivator-1alpha was also significantly decreased 14 d after myostatin gene electrotransfer .
	manualset3
218381	1	420258	7	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This study therefore shows that lupus activity may persist in patients with ESRD .
	manualset3
218382	2	420258	7	NULL	NULL	0	NULL	lupus activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This study therefore shows that lupus activity may persist in patients with ESRD .
	manualset3
218383	3	420258	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This study therefore shows that lupus activity may persist in patients with ESRD .
	manualset3
218384	4	420258	7	NULL	NULL	0	NULL	ESRD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This study therefore shows that lupus activity may persist in patients with ESRD .
	manualset3
218385	1	420259	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these results replicate earlier findings about the genetic background of SZ-ND and SZ-D only partially , our data seem to confirm previously reported association of NRG1 with schizophrenia without prominent negative symptoms .
	manualset3
218386	2	420259	7	NULL	NULL	0	NULL	earlier findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these results replicate earlier findings about the genetic background of SZ-ND and SZ-D only partially , our data seem to confirm previously reported association of NRG1 with schizophrenia without prominent negative symptoms .
	manualset3
218387	3	420259	7	NULL	NULL	0	NULL	genetic background	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these results replicate earlier findings about the genetic background of SZ-ND and SZ-D only partially , our data seem to confirm previously reported association of NRG1 with schizophrenia without prominent negative symptoms .
	manualset3
218388	4	420259	7	NULL	NULL	0	NULL	SZ-ND 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these results replicate earlier findings about the genetic background of SZ-ND and SZ-D only partially , our data seem to confirm previously reported association of NRG1 with schizophrenia without prominent negative symptoms .
	manualset3
218389	5	420259	7	NULL	NULL	0	NULL	SZ-D	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these results replicate earlier findings about the genetic background of SZ-ND and SZ-D only partially , our data seem to confirm previously reported association of NRG1 with schizophrenia without prominent negative symptoms .
	manualset3
218390	6	420259	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these results replicate earlier findings about the genetic background of SZ-ND and SZ-D only partially , our data seem to confirm previously reported association of NRG1 with schizophrenia without prominent negative symptoms .
	manualset3
218391	7	420259	7	NULL	NULL	NULL	NULL	association 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although these results replicate earlier findings about the genetic background of SZ-ND and SZ-D only partially , our data seem to confirm previously reported association of NRG1 with schizophrenia without prominent negative symptoms .
	manualset3
218392	8	420259	7	NULL	NULL	0	NULL	NRG1	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these results replicate earlier findings about the genetic background of SZ-ND and SZ-D only partially , our data seem to confirm previously reported association of NRG1 with schizophrenia without prominent negative symptoms .
	manualset3
218393	9	420259	7	NULL	NULL	0	NULL	schizophrenia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these results replicate earlier findings about the genetic background of SZ-ND and SZ-D only partially , our data seem to confirm previously reported association of NRG1 with schizophrenia without prominent negative symptoms .
	manualset3
218394	10	420259	7	NULL	NULL	0	NULL	negative symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these results replicate earlier findings about the genetic background of SZ-ND and SZ-D only partially , our data seem to confirm previously reported association of NRG1 with schizophrenia without prominent negative symptoms .
	manualset3
218395	1	420260	7	NULL	NULL	0	NULL	Analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of parotid and mixed saliva in Roe deer ( Capreolus capreolus L. ) .
	manualset3
218396	2	420260	7	NULL	NULL	0	NULL	parotid	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of parotid and mixed saliva in Roe deer ( Capreolus capreolus L. ) .
	manualset3
218397	3	420260	7	NULL	NULL	0	NULL	mixed saliva	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of parotid and mixed saliva in Roe deer ( Capreolus capreolus L. ) .
	manualset3
218398	4	420260	7	NULL	NULL	0	NULL	Roe deer	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of parotid and mixed saliva in Roe deer ( Capreolus capreolus L. ) .
	manualset3
218399	5	420260	7	NULL	NULL	0	NULL	Capreolus capreolus L	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of parotid and mixed saliva in Roe deer ( Capreolus capreolus L. ) .
	manualset3
218400	1	420261	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that 99mTc-MAG3 is a useful and clinically applicable radiopharmaceutical for measurement of effective renal blood flow in the horse .
	manualset3
218401	2	420261	7	NULL	NULL	0	NULL	99mTc-MAG3	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that 99mTc-MAG3 is a useful and clinically applicable radiopharmaceutical for measurement of effective renal blood flow in the horse .
	manualset3
218402	3	420261	7	NULL	NULL	0	NULL	radiopharmaceutical	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that 99mTc-MAG3 is a useful and clinically applicable radiopharmaceutical for measurement of effective renal blood flow in the horse .
	manualset3
218403	4	420261	7	NULL	NULL	0	NULL	measurement	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that 99mTc-MAG3 is a useful and clinically applicable radiopharmaceutical for measurement of effective renal blood flow in the horse .
	manualset3
218404	5	420261	7	NULL	NULL	0	NULL	effective renal blood flow	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that 99mTc-MAG3 is a useful and clinically applicable radiopharmaceutical for measurement of effective renal blood flow in the horse .
	manualset3
218405	6	420261	7	NULL	NULL	0	NULL	horse	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that 99mTc-MAG3 is a useful and clinically applicable radiopharmaceutical for measurement of effective renal blood flow in the horse .
	manualset3
218406	1	420262	7	NULL	NULL	0	NULL	pathfinding	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	During pathfinding , motoneuronal growth cones encounter three distinct regions : a common pathway , a choice point , and separate cell-specific pathways .
	manualset3
218407	2	420262	7	NULL	NULL	0	NULL	motoneuronal growth cones	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	During pathfinding , motoneuronal growth cones encounter three distinct regions : a common pathway , a choice point , and separate cell-specific pathways .
	manualset3
218408	3	420262	7	NULL	NULL	0	NULL	three distinct regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	During pathfinding , motoneuronal growth cones encounter three distinct regions : a common pathway , a choice point , and separate cell-specific pathways .
	manualset3
218409	4	420262	7	NULL	NULL	NULL	NULL	common pathway	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During pathfinding , motoneuronal growth cones encounter three distinct regions : a common pathway , a choice point , and separate cell-specific pathways .
	manualset3
218410	5	420262	7	NULL	NULL	NULL	NULL	choice point 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During pathfinding , motoneuronal growth cones encounter three distinct regions : a common pathway , a choice point , and separate cell-specific pathways .
	manualset3
218411	6	420262	7	NULL	NULL	NULL	NULL	cell-specific pathways	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During pathfinding , motoneuronal growth cones encounter three distinct regions : a common pathway , a choice point , and separate cell-specific pathways .
	manualset3
218412	1	420263	7	NULL	NULL	0	NULL	acyl-CoA-independent TAG synthase activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , we unveiled an acyl-CoA-independent TAG synthase activity in lipid particles which is distinct from Dga1p and the phosphatidylcholine : DAGAT Lro1p .
	manualset3
218413	2	420263	7	NULL	NULL	0	NULL	 lipid particles	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , we unveiled an acyl-CoA-independent TAG synthase activity in lipid particles which is distinct from Dga1p and the phosphatidylcholine : DAGAT Lro1p .
	manualset3
218414	3	420263	7	NULL	NULL	0	NULL	Dga1p	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , we unveiled an acyl-CoA-independent TAG synthase activity in lipid particles which is distinct from Dga1p and the phosphatidylcholine : DAGAT Lro1p .
	manualset3
218415	4	420263	7	NULL	NULL	0	NULL	phosphatidylcholine : DAGAT Lro1p	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , we unveiled an acyl-CoA-independent TAG synthase activity in lipid particles which is distinct from Dga1p and the phosphatidylcholine : DAGAT Lro1p .
	manualset3
218416	1	420264	7	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of developing cancer after solid organ transplantation ( SOT ) is about 5 - to 10-fold greater than that of the general population .
	manualset3
218417	2	420264	7	NULL	NULL	0	NULL	 developing cancer	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of developing cancer after solid organ transplantation ( SOT ) is about 5 - to 10-fold greater than that of the general population .
	manualset3
218418	3	420264	7	NULL	NULL	0	NULL	solid organ transplantation ( SOT )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of developing cancer after solid organ transplantation ( SOT ) is about 5 - to 10-fold greater than that of the general population .
	manualset3
218419	4	420264	7	NULL	NULL	0	NULL	5 - to 10-fold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of developing cancer after solid organ transplantation ( SOT ) is about 5 - to 10-fold greater than that of the general population .
	manualset3
218420	5	420264	7	NULL	NULL	0	NULL	general population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of developing cancer after solid organ transplantation ( SOT ) is about 5 - to 10-fold greater than that of the general population .
	manualset3
218421	1	420265	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , one of the examined SNPs ( rs981782 in HCN1 ) had a protective effect that was significantly stronger in premenopausal women ( P-value : 7.9 10 ( -4 ) ) .
	manualset3
218422	2	420265	7	NULL	NULL	0	NULL	SNPs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , one of the examined SNPs ( rs981782 in HCN1 ) had a protective effect that was significantly stronger in premenopausal women ( P-value : 7.9 10 ( -4 ) ) .
	manualset3
218423	3	420265	7	NULL	NULL	0	NULL	 rs981782	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , one of the examined SNPs ( rs981782 in HCN1 ) had a protective effect that was significantly stronger in premenopausal women ( P-value : 7.9 10 ( -4 ) ) .
	manualset3
218424	4	420265	7	NULL	NULL	0	NULL	HCN1	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , one of the examined SNPs ( rs981782 in HCN1 ) had a protective effect that was significantly stronger in premenopausal women ( P-value : 7.9 10 ( -4 ) ) .
	manualset3
218425	5	420265	7	NULL	NULL	0	NULL	protective effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , one of the examined SNPs ( rs981782 in HCN1 ) had a protective effect that was significantly stronger in premenopausal women ( P-value : 7.9 10 ( -4 ) ) .
	manualset3
218426	6	420265	7	NULL	NULL	0	NULL	premenopausal women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , one of the examined SNPs ( rs981782 in HCN1 ) had a protective effect that was significantly stronger in premenopausal women ( P-value : 7.9 10 ( -4 ) ) .
	manualset3
218427	7	420265	7	NULL	NULL	0	NULL	P-value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , one of the examined SNPs ( rs981782 in HCN1 ) had a protective effect that was significantly stronger in premenopausal women ( P-value : 7.9 10 ( -4 ) ) .
	manualset3
218428	8	420265	7	NULL	NULL	0	NULL	7.9 10 ( -4 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , one of the examined SNPs ( rs981782 in HCN1 ) had a protective effect that was significantly stronger in premenopausal women ( P-value : 7.9 10 ( -4 ) ) .
	manualset3
218429	1	420266	7	NULL	NULL	0	NULL	Human rabies encephalitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Human rabies encephalitis by a vampire bat bite in an urban area of Colombia A case of rabies encephalitis is presented in a teenaged male , which developed four months after a bat bite in the urban area of Floridablanca , Santander Province , Colombia .
	manualset3
218430	2	420266	7	NULL	NULL	0	NULL	 vampire bat bite	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Human rabies encephalitis by a vampire bat bite in an urban area of Colombia A case of rabies encephalitis is presented in a teenaged male , which developed four months after a bat bite in the urban area of Floridablanca , Santander Province , Colombia .
	manualset3
218431	3	420266	7	NULL	NULL	NULL	NULL	urban area	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human rabies encephalitis by a vampire bat bite in an urban area of Colombia A case of rabies encephalitis is presented in a teenaged male , which developed four months after a bat bite in the urban area of Floridablanca , Santander Province , Colombia .
	manualset3
218432	4	420266	7	NULL	NULL	0	NULL	Colombia 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Human rabies encephalitis by a vampire bat bite in an urban area of Colombia A case of rabies encephalitis is presented in a teenaged male , which developed four months after a bat bite in the urban area of Floridablanca , Santander Province , Colombia .
	manualset3
218433	5	420266	7	NULL	NULL	0	NULL	case	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Human rabies encephalitis by a vampire bat bite in an urban area of Colombia A case of rabies encephalitis is presented in a teenaged male , which developed four months after a bat bite in the urban area of Floridablanca , Santander Province , Colombia .
	manualset3
218434	6	420266	7	NULL	NULL	0	NULL	rabies encephalitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Human rabies encephalitis by a vampire bat bite in an urban area of Colombia A case of rabies encephalitis is presented in a teenaged male , which developed four months after a bat bite in the urban area of Floridablanca , Santander Province , Colombia .
	manualset3
218435	7	420266	7	NULL	NULL	0	NULL	teenaged male	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Human rabies encephalitis by a vampire bat bite in an urban area of Colombia A case of rabies encephalitis is presented in a teenaged male , which developed four months after a bat bite in the urban area of Floridablanca , Santander Province , Colombia .
	manualset3
218436	8	420266	7	NULL	NULL	0	NULL	four months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Human rabies encephalitis by a vampire bat bite in an urban area of Colombia A case of rabies encephalitis is presented in a teenaged male , which developed four months after a bat bite in the urban area of Floridablanca , Santander Province , Colombia .
	manualset3
218437	9	420266	7	NULL	NULL	0	NULL	 bat bite	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Human rabies encephalitis by a vampire bat bite in an urban area of Colombia A case of rabies encephalitis is presented in a teenaged male , which developed four months after a bat bite in the urban area of Floridablanca , Santander Province , Colombia .
	manualset3
218438	10	420266	7	NULL	NULL	0	NULL	urban area	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Human rabies encephalitis by a vampire bat bite in an urban area of Colombia A case of rabies encephalitis is presented in a teenaged male , which developed four months after a bat bite in the urban area of Floridablanca , Santander Province , Colombia .
	manualset3
218439	11	420266	7	NULL	NULL	0	NULL	Floridablanca	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Human rabies encephalitis by a vampire bat bite in an urban area of Colombia A case of rabies encephalitis is presented in a teenaged male , which developed four months after a bat bite in the urban area of Floridablanca , Santander Province , Colombia .
	manualset3
218440	12	420266	7	NULL	NULL	0	NULL	Santander Province	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Human rabies encephalitis by a vampire bat bite in an urban area of Colombia A case of rabies encephalitis is presented in a teenaged male , which developed four months after a bat bite in the urban area of Floridablanca , Santander Province , Colombia .
	manualset3
218441	13	420266	7	NULL	NULL	0	NULL	Colombia	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Human rabies encephalitis by a vampire bat bite in an urban area of Colombia A case of rabies encephalitis is presented in a teenaged male , which developed four months after a bat bite in the urban area of Floridablanca , Santander Province , Colombia .
	manualset3
218442	1	420267	7	NULL	NULL	0	NULL	Death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Death due to acute pancreatitis after endoscopic retrograde cholangiography ) .
	manualset3
218443	2	420267	7	NULL	NULL	0	NULL	acute pancreatitis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Death due to acute pancreatitis after endoscopic retrograde cholangiography ) .
	manualset3
218444	3	420267	7	NULL	NULL	0	NULL	endoscopic retrograde cholangiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Death due to acute pancreatitis after endoscopic retrograde cholangiography ) .
	manualset3
218445	1	420268	7	NULL	NULL	0	NULL	 Web-based resource	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this Web-based resource was created in response to federal requirements for education in human subjects protection , the author 's evaluation suggests that learners value and respond to the content in ways that transcend mere compliance .
	manualset3
218446	2	420268	7	NULL	NULL	0	NULL	response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this Web-based resource was created in response to federal requirements for education in human subjects protection , the author 's evaluation suggests that learners value and respond to the content in ways that transcend mere compliance .
	manualset3
218447	3	420268	7	NULL	NULL	0	NULL	federal requirements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this Web-based resource was created in response to federal requirements for education in human subjects protection , the author 's evaluation suggests that learners value and respond to the content in ways that transcend mere compliance .
	manualset3
218448	4	420268	7	NULL	NULL	NULL	NULL	education	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although this Web-based resource was created in response to federal requirements for education in human subjects protection , the author 's evaluation suggests that learners value and respond to the content in ways that transcend mere compliance .
	manualset3
218449	5	420268	7	NULL	NULL	0	NULL	human subjects protection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this Web-based resource was created in response to federal requirements for education in human subjects protection , the author 's evaluation suggests that learners value and respond to the content in ways that transcend mere compliance .
	manualset3
218450	6	420268	7	NULL	NULL	0	NULL	author 's evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this Web-based resource was created in response to federal requirements for education in human subjects protection , the author 's evaluation suggests that learners value and respond to the content in ways that transcend mere compliance .
	manualset3
218451	7	420268	7	NULL	NULL	0	NULL	learners	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this Web-based resource was created in response to federal requirements for education in human subjects protection , the author 's evaluation suggests that learners value and respond to the content in ways that transcend mere compliance .
	manualset3
218452	8	420268	7	NULL	NULL	0	NULL	content	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this Web-based resource was created in response to federal requirements for education in human subjects protection , the author 's evaluation suggests that learners value and respond to the content in ways that transcend mere compliance .
	manualset3
218453	9	420268	7	NULL	NULL	0	NULL	ways	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this Web-based resource was created in response to federal requirements for education in human subjects protection , the author 's evaluation suggests that learners value and respond to the content in ways that transcend mere compliance .
	manualset3
218454	10	420268	7	NULL	NULL	0	NULL	compliance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this Web-based resource was created in response to federal requirements for education in human subjects protection , the author 's evaluation suggests that learners value and respond to the content in ways that transcend mere compliance .
	manualset3
218455	1	420269	7	NULL	NULL	0	NULL	cytokine levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytokine levels could be further increased by the novel protein kinase C agonist PEP005 , which also induced significant production of IL2 and TNFalpha which could contribute to anti-tumor effects in AML patients .
	manualset3
218456	2	420269	7	NULL	NULL	0	NULL	novel protein kinase C agonist PEP005	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytokine levels could be further increased by the novel protein kinase C agonist PEP005 , which also induced significant production of IL2 and TNFalpha which could contribute to anti-tumor effects in AML patients .
	manualset3
218457	3	420269	7	NULL	NULL	0	NULL	production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytokine levels could be further increased by the novel protein kinase C agonist PEP005 , which also induced significant production of IL2 and TNFalpha which could contribute to anti-tumor effects in AML patients .
	manualset3
218458	4	420269	7	NULL	NULL	0	NULL	IL2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytokine levels could be further increased by the novel protein kinase C agonist PEP005 , which also induced significant production of IL2 and TNFalpha which could contribute to anti-tumor effects in AML patients .
	manualset3
218459	5	420269	7	NULL	NULL	0	NULL	TNFalpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytokine levels could be further increased by the novel protein kinase C agonist PEP005 , which also induced significant production of IL2 and TNFalpha which could contribute to anti-tumor effects in AML patients .
	manualset3
218460	6	420269	7	NULL	NULL	0	NULL	anti-tumor effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytokine levels could be further increased by the novel protein kinase C agonist PEP005 , which also induced significant production of IL2 and TNFalpha which could contribute to anti-tumor effects in AML patients .
	manualset3
218461	7	420269	7	NULL	NULL	0	NULL	AML patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The cytokine levels could be further increased by the novel protein kinase C agonist PEP005 , which also induced significant production of IL2 and TNFalpha which could contribute to anti-tumor effects in AML patients .
	manualset3
218462	1	420270	7	NULL	NULL	NULL	NULL	expansion	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although significant expansion of bone marrow cultures occurred in the presence and absence of human stroma , the results of expansion were effectively better in the presence of a stromal layer .
	manualset3
218463	2	420270	7	NULL	NULL	0	NULL	bone marrow cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Although significant expansion of bone marrow cultures occurred in the presence and absence of human stroma , the results of expansion were effectively better in the presence of a stromal layer .
	manualset3
218464	3	420270	7	NULL	NULL	0	NULL	human stroma	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Although significant expansion of bone marrow cultures occurred in the presence and absence of human stroma , the results of expansion were effectively better in the presence of a stromal layer .
	manualset3
218465	4	420270	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although significant expansion of bone marrow cultures occurred in the presence and absence of human stroma , the results of expansion were effectively better in the presence of a stromal layer .
	manualset3
218466	5	420270	7	NULL	NULL	0	NULL	expansion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although significant expansion of bone marrow cultures occurred in the presence and absence of human stroma , the results of expansion were effectively better in the presence of a stromal layer .
	manualset3
218467	6	420270	7	NULL	NULL	0	NULL	stromal layer	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Although significant expansion of bone marrow cultures occurred in the presence and absence of human stroma , the results of expansion were effectively better in the presence of a stromal layer .
	manualset3
218468	1	420271	7	NULL	NULL	0	NULL	Two `` private polymorphisms '	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two `` private polymorphisms '' were encountered , of PEPB in the Pano and CAII in the Baniwa .
	manualset3
218469	2	420271	7	NULL	NULL	0	NULL	PEPB	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Two `` private polymorphisms '' were encountered , of PEPB in the Pano and CAII in the Baniwa .
	manualset3
218470	3	420271	7	NULL	NULL	0	NULL	Pano	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two `` private polymorphisms '' were encountered , of PEPB in the Pano and CAII in the Baniwa .
	manualset3
218471	4	420271	7	NULL	NULL	0	NULL	CAII	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two `` private polymorphisms '' were encountered , of PEPB in the Pano and CAII in the Baniwa .
	manualset3
218472	5	420271	7	NULL	NULL	0	NULL	Baniwa	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two `` private polymorphisms '' were encountered , of PEPB in the Pano and CAII in the Baniwa .
	manualset3
218473	1	420272	7	NULL	NULL	0	NULL	California	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In California , however , where the medical and dental professions are not trusted to put their own house in order , everything is covered by legislation and becomes the subject of intense political lobbying .
	manualset3
218474	2	420272	7	NULL	NULL	0	NULL	medical professions	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In California , however , where the medical and dental professions are not trusted to put their own house in order , everything is covered by legislation and becomes the subject of intense political lobbying .
	manualset3
218475	3	420272	7	NULL	NULL	0	NULL	dental professions	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In California , however , where the medical and dental professions are not trusted to put their own house in order , everything is covered by legislation and becomes the subject of intense political lobbying .
	manualset3
218476	4	420272	7	NULL	NULL	0	NULL	house	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In California , however , where the medical and dental professions are not trusted to put their own house in order , everything is covered by legislation and becomes the subject of intense political lobbying .
	manualset3
218477	5	420272	7	NULL	NULL	0	NULL	legislation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In California , however , where the medical and dental professions are not trusted to put their own house in order , everything is covered by legislation and becomes the subject of intense political lobbying .
	manualset3
218478	6	420272	7	NULL	NULL	0	NULL	subject	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In California , however , where the medical and dental professions are not trusted to put their own house in order , everything is covered by legislation and becomes the subject of intense political lobbying .
	manualset3
218479	7	420272	7	NULL	NULL	0	NULL	 intense political lobbying 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In California , however , where the medical and dental professions are not trusted to put their own house in order , everything is covered by legislation and becomes the subject of intense political lobbying .
	manualset3
218480	1	420273	7	NULL	NULL	0	NULL	holographic technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The holographic technique detects mainly the activity on the surface and is applicable to assessment of the early drying process of paint .
	manualset3
218481	2	420273	7	NULL	NULL	0	NULL	activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The holographic technique detects mainly the activity on the surface and is applicable to assessment of the early drying process of paint .
	manualset3
218482	3	420273	7	NULL	NULL	0	NULL	surface	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The holographic technique detects mainly the activity on the surface and is applicable to assessment of the early drying process of paint .
	manualset3
218483	4	420273	7	NULL	NULL	0	NULL	assessment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The holographic technique detects mainly the activity on the surface and is applicable to assessment of the early drying process of paint .
	manualset3
218484	5	420273	7	NULL	NULL	0	NULL	early drying process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The holographic technique detects mainly the activity on the surface and is applicable to assessment of the early drying process of paint .
	manualset3
218485	6	420273	7	NULL	NULL	0	NULL	 paint	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The holographic technique detects mainly the activity on the surface and is applicable to assessment of the early drying process of paint .
	manualset3
218486	1	420274	7	NULL	NULL	0	NULL	Competitive interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive interactions between L-alanine and L-phenylalanine in rabbit ileum .
	manualset3
218487	2	420274	7	NULL	NULL	0	NULL	L-alanine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive interactions between L-alanine and L-phenylalanine in rabbit ileum .
	manualset3
218488	3	420274	7	NULL	NULL	0	NULL	L-phenylalanine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive interactions between L-alanine and L-phenylalanine in rabbit ileum .
	manualset3
218489	4	420274	7	NULL	NULL	0	NULL	rabbit ileum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive interactions between L-alanine and L-phenylalanine in rabbit ileum .
	manualset3
218490	1	420275	7	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no correlation between the volume density of lysosomes and either the duration of postmortem anoxia , clinical course , or patient 's age .
	manualset3
218491	2	420275	7	NULL	NULL	0	NULL	volume density	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no correlation between the volume density of lysosomes and either the duration of postmortem anoxia , clinical course , or patient 's age .
	manualset3
218492	3	420275	7	NULL	NULL	0	NULL	 lysosomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no correlation between the volume density of lysosomes and either the duration of postmortem anoxia , clinical course , or patient 's age .
	manualset3
218493	4	420275	7	NULL	NULL	0	NULL	duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no correlation between the volume density of lysosomes and either the duration of postmortem anoxia , clinical course , or patient 's age .
	manualset3
218494	5	420275	7	NULL	NULL	0	NULL	postmortem anoxia	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no correlation between the volume density of lysosomes and either the duration of postmortem anoxia , clinical course , or patient 's age .
	manualset3
218495	6	420275	7	NULL	NULL	NULL	NULL	clinical course 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There was no correlation between the volume density of lysosomes and either the duration of postmortem anoxia , clinical course , or patient 's age .
	manualset3
218496	7	420275	7	NULL	NULL	0	NULL	patient 's age	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no correlation between the volume density of lysosomes and either the duration of postmortem anoxia , clinical course , or patient 's age .
	manualset3
218497	1	420276	7	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the downstream effectors of c-Src is Akt1 .
	manualset3
218498	2	420276	7	NULL	NULL	0	NULL	downstream effectors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the downstream effectors of c-Src is Akt1 .
	manualset3
218499	3	420276	7	NULL	NULL	0	NULL	c-Src	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the downstream effectors of c-Src is Akt1 .
	manualset3
218500	4	420276	7	NULL	NULL	0	NULL	Akt1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the downstream effectors of c-Src is Akt1 .
	manualset3
218501	1	420277	7	NULL	NULL	0	NULL	cytosolic detoxification enzyme	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this is a cytosolic detoxification enzyme , the pH optimum for the standard assay substrate 4-nitrophenol is at pH 5.5 ; upon oxidation , the optimum changes to the physiological pH range .
	manualset3
218502	2	420277	7	NULL	NULL	0	NULL	pH optimum	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this is a cytosolic detoxification enzyme , the pH optimum for the standard assay substrate 4-nitrophenol is at pH 5.5 ; upon oxidation , the optimum changes to the physiological pH range .
	manualset3
218503	3	420277	7	NULL	NULL	NULL	NULL	standard assay substrate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although this is a cytosolic detoxification enzyme , the pH optimum for the standard assay substrate 4-nitrophenol is at pH 5.5 ; upon oxidation , the optimum changes to the physiological pH range .
	manualset3
218504	4	420277	7	NULL	NULL	0	NULL	4-nitrophenol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this is a cytosolic detoxification enzyme , the pH optimum for the standard assay substrate 4-nitrophenol is at pH 5.5 ; upon oxidation , the optimum changes to the physiological pH range .
	manualset3
218505	5	420277	7	NULL	NULL	0	NULL	pH 5.5	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this is a cytosolic detoxification enzyme , the pH optimum for the standard assay substrate 4-nitrophenol is at pH 5.5 ; upon oxidation , the optimum changes to the physiological pH range .
	manualset3
218506	6	420277	7	NULL	NULL	0	NULL	oxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this is a cytosolic detoxification enzyme , the pH optimum for the standard assay substrate 4-nitrophenol is at pH 5.5 ; upon oxidation , the optimum changes to the physiological pH range .
	manualset3
218507	7	420277	7	NULL	NULL	NULL	NULL	optimum	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although this is a cytosolic detoxification enzyme , the pH optimum for the standard assay substrate 4-nitrophenol is at pH 5.5 ; upon oxidation , the optimum changes to the physiological pH range .
	manualset3
218508	8	420277	7	NULL	NULL	0	NULL	physiological pH range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this is a cytosolic detoxification enzyme , the pH optimum for the standard assay substrate 4-nitrophenol is at pH 5.5 ; upon oxidation , the optimum changes to the physiological pH range .
	manualset3
218509	1	420278	7	NULL	NULL	0	NULL	Ventriculography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ventriculography with meglumine iocarmate ( Dimer X ) or Metrizamide ( Amipaque was carried out in 15 infants with myelomeningocele and progressive hydrocephalus .
	manualset3
218510	2	420278	7	NULL	NULL	0	NULL	meglumine iocarmate ( Dimer X )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Ventriculography with meglumine iocarmate ( Dimer X ) or Metrizamide ( Amipaque was carried out in 15 infants with myelomeningocele and progressive hydrocephalus .
	manualset3
218511	3	420278	7	NULL	NULL	0	NULL	Metrizamide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Ventriculography with meglumine iocarmate ( Dimer X ) or Metrizamide ( Amipaque was carried out in 15 infants with myelomeningocele and progressive hydrocephalus .
	manualset3
218512	4	420278	7	NULL	NULL	0	NULL	Amipaque	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Ventriculography with meglumine iocarmate ( Dimer X ) or Metrizamide ( Amipaque was carried out in 15 infants with myelomeningocele and progressive hydrocephalus .
	manualset3
218513	5	420278	7	NULL	NULL	0	NULL	15 infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ventriculography with meglumine iocarmate ( Dimer X ) or Metrizamide ( Amipaque was carried out in 15 infants with myelomeningocele and progressive hydrocephalus .
	manualset3
218514	6	420278	7	NULL	NULL	0	NULL	myelomeningocele	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Ventriculography with meglumine iocarmate ( Dimer X ) or Metrizamide ( Amipaque was carried out in 15 infants with myelomeningocele and progressive hydrocephalus .
	manualset3
218515	7	420278	7	NULL	NULL	0	NULL	progressive hydrocephalus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Ventriculography with meglumine iocarmate ( Dimer X ) or Metrizamide ( Amipaque was carried out in 15 infants with myelomeningocele and progressive hydrocephalus .
	manualset3
218516	1	420279	7	NULL	NULL	0	NULL	 levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we found that levels of AC6 mRNA , the most highly expressed AC isoform in the inner medulla , inversely correlate with fluid intake .
	manualset3
218517	2	420279	7	NULL	NULL	0	NULL	AC6 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we found that levels of AC6 mRNA , the most highly expressed AC isoform in the inner medulla , inversely correlate with fluid intake .
	manualset3
218518	3	420279	7	NULL	NULL	0	NULL	AC isoform 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we found that levels of AC6 mRNA , the most highly expressed AC isoform in the inner medulla , inversely correlate with fluid intake .
	manualset3
218520	4	420279	7	NULL	NULL	0	NULL	inner medulla	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we found that levels of AC6 mRNA , the most highly expressed AC isoform in the inner medulla , inversely correlate with fluid intake .
	manualset3
218521	5	420279	7	NULL	NULL	0	NULL	fluid intake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we found that levels of AC6 mRNA , the most highly expressed AC isoform in the inner medulla , inversely correlate with fluid intake .
	manualset3
218522	1	420280	7	NULL	NULL	0	NULL	Stroke patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Stroke patients ( without SDB ) have reductions in total sleep time and sleep efficiency , reduced stage II and slow wave sleep , increased wakefulness during sleep and increased sleep latency .
	manualset3
218523	2	420280	7	NULL	NULL	0	NULL	SDB	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Stroke patients ( without SDB ) have reductions in total sleep time and sleep efficiency , reduced stage II and slow wave sleep , increased wakefulness during sleep and increased sleep latency .
	manualset3
218524	3	420280	7	NULL	NULL	0	NULL	reductions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stroke patients ( without SDB ) have reductions in total sleep time and sleep efficiency , reduced stage II and slow wave sleep , increased wakefulness during sleep and increased sleep latency .
	manualset3
218525	4	420280	7	NULL	NULL	0	NULL	total sleep time	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Stroke patients ( without SDB ) have reductions in total sleep time and sleep efficiency , reduced stage II and slow wave sleep , increased wakefulness during sleep and increased sleep latency .
	manualset3
218526	5	420280	7	NULL	NULL	0	NULL	 sleep efficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Stroke patients ( without SDB ) have reductions in total sleep time and sleep efficiency , reduced stage II and slow wave sleep , increased wakefulness during sleep and increased sleep latency .
	manualset3
218527	6	420280	7	NULL	NULL	0	NULL	reduced stage II	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Stroke patients ( without SDB ) have reductions in total sleep time and sleep efficiency , reduced stage II and slow wave sleep , increased wakefulness during sleep and increased sleep latency .
	manualset3
218528	7	420280	7	NULL	NULL	0	NULL	slow wave sleep	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Stroke patients ( without SDB ) have reductions in total sleep time and sleep efficiency , reduced stage II and slow wave sleep , increased wakefulness during sleep and increased sleep latency .
	manualset3
218529	8	420280	7	NULL	NULL	0	NULL	wakefulness 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stroke patients ( without SDB ) have reductions in total sleep time and sleep efficiency , reduced stage II and slow wave sleep , increased wakefulness during sleep and increased sleep latency .
	manualset3
218530	9	420280	7	NULL	NULL	0	NULL	sleep	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stroke patients ( without SDB ) have reductions in total sleep time and sleep efficiency , reduced stage II and slow wave sleep , increased wakefulness during sleep and increased sleep latency .
	manualset3
218531	10	420280	7	NULL	NULL	0	NULL	sleep latency 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Stroke patients ( without SDB ) have reductions in total sleep time and sleep efficiency , reduced stage II and slow wave sleep , increased wakefulness during sleep and increased sleep latency .
	manualset3
218532	1	420281	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using one particulate zinc oxide ( ZnO ) and two soluble zinc compounds ( Zn ( NO ( 3 ) ) ( 2 ) and Zn ( CH ( 3 ) COO ) ( 2 ) ) , we aimed to clarify if zinc ions ( Zn ( 2 + ) ) , like particulate ZnO , caused inflammatory responses in vascular endothelial cells .
	manualset3
218533	2	420281	7	NULL	NULL	0	NULL	 zinc oxide ( ZnO )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using one particulate zinc oxide ( ZnO ) and two soluble zinc compounds ( Zn ( NO ( 3 ) ) ( 2 ) and Zn ( CH ( 3 ) COO ) ( 2 ) ) , we aimed to clarify if zinc ions ( Zn ( 2 + ) ) , like particulate ZnO , caused inflammatory responses in vascular endothelial cells .
	manualset3
218534	3	420281	7	NULL	NULL	0	NULL	two soluble zinc compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using one particulate zinc oxide ( ZnO ) and two soluble zinc compounds ( Zn ( NO ( 3 ) ) ( 2 ) and Zn ( CH ( 3 ) COO ) ( 2 ) ) , we aimed to clarify if zinc ions ( Zn ( 2 + ) ) , like particulate ZnO , caused inflammatory responses in vascular endothelial cells .
	manualset3
218535	4	420281	7	NULL	NULL	0	NULL	( Zn ( NO ( 3 ) ) ( 2 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using one particulate zinc oxide ( ZnO ) and two soluble zinc compounds ( Zn ( NO ( 3 ) ) ( 2 ) and Zn ( CH ( 3 ) COO ) ( 2 ) ) , we aimed to clarify if zinc ions ( Zn ( 2 + ) ) , like particulate ZnO , caused inflammatory responses in vascular endothelial cells .
	manualset3
218536	5	420281	7	NULL	NULL	0	NULL	Zn ( CH ( 3 ) COO ) ( 2 ) )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using one particulate zinc oxide ( ZnO ) and two soluble zinc compounds ( Zn ( NO ( 3 ) ) ( 2 ) and Zn ( CH ( 3 ) COO ) ( 2 ) ) , we aimed to clarify if zinc ions ( Zn ( 2 + ) ) , like particulate ZnO , caused inflammatory responses in vascular endothelial cells .
	manualset3
218537	6	420281	7	NULL	NULL	0	NULL	zinc ions ( Zn ( 2 + ) )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Using one particulate zinc oxide ( ZnO ) and two soluble zinc compounds ( Zn ( NO ( 3 ) ) ( 2 ) and Zn ( CH ( 3 ) COO ) ( 2 ) ) , we aimed to clarify if zinc ions ( Zn ( 2 + ) ) , like particulate ZnO , caused inflammatory responses in vascular endothelial cells .
	manualset3
218538	7	420281	7	NULL	NULL	0	NULL	ZnO 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using one particulate zinc oxide ( ZnO ) and two soluble zinc compounds ( Zn ( NO ( 3 ) ) ( 2 ) and Zn ( CH ( 3 ) COO ) ( 2 ) ) , we aimed to clarify if zinc ions ( Zn ( 2 + ) ) , like particulate ZnO , caused inflammatory responses in vascular endothelial cells .
	manualset3
218539	8	420281	7	NULL	NULL	0	NULL	inflammatory responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using one particulate zinc oxide ( ZnO ) and two soluble zinc compounds ( Zn ( NO ( 3 ) ) ( 2 ) and Zn ( CH ( 3 ) COO ) ( 2 ) ) , we aimed to clarify if zinc ions ( Zn ( 2 + ) ) , like particulate ZnO , caused inflammatory responses in vascular endothelial cells .
	manualset3
218540	9	420281	7	NULL	NULL	0	NULL	vascular endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using one particulate zinc oxide ( ZnO ) and two soluble zinc compounds ( Zn ( NO ( 3 ) ) ( 2 ) and Zn ( CH ( 3 ) COO ) ( 2 ) ) , we aimed to clarify if zinc ions ( Zn ( 2 + ) ) , like particulate ZnO , caused inflammatory responses in vascular endothelial cells .
	manualset3
218541	1	420282	7	NULL	NULL	0	NULL	 effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of several variables on nanoparticle characteristics was evaluated , including the ratio of drug-polymer , the amount of the poly vinyl alcohol as surfactant , and the internal phase volume/composition .
	manualset3
218542	2	420282	7	NULL	NULL	0	NULL	several variables	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of several variables on nanoparticle characteristics was evaluated , including the ratio of drug-polymer , the amount of the poly vinyl alcohol as surfactant , and the internal phase volume/composition .
	manualset3
218543	3	420282	7	NULL	NULL	0	NULL	nanoparticle characteristics 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of several variables on nanoparticle characteristics was evaluated , including the ratio of drug-polymer , the amount of the poly vinyl alcohol as surfactant , and the internal phase volume/composition .
	manualset3
218544	4	420282	7	NULL	NULL	0	NULL	ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of several variables on nanoparticle characteristics was evaluated , including the ratio of drug-polymer , the amount of the poly vinyl alcohol as surfactant , and the internal phase volume/composition .
	manualset3
218545	5	420282	7	NULL	NULL	0	NULL	drug-polymer	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of several variables on nanoparticle characteristics was evaluated , including the ratio of drug-polymer , the amount of the poly vinyl alcohol as surfactant , and the internal phase volume/composition .
	manualset3
218546	6	420282	7	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of several variables on nanoparticle characteristics was evaluated , including the ratio of drug-polymer , the amount of the poly vinyl alcohol as surfactant , and the internal phase volume/composition .
	manualset3
218547	7	420282	7	NULL	NULL	0	NULL	poly vinyl alcohol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of several variables on nanoparticle characteristics was evaluated , including the ratio of drug-polymer , the amount of the poly vinyl alcohol as surfactant , and the internal phase volume/composition .
	manualset3
218548	8	420282	7	NULL	NULL	0	NULL	surfactant	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of several variables on nanoparticle characteristics was evaluated , including the ratio of drug-polymer , the amount of the poly vinyl alcohol as surfactant , and the internal phase volume/composition .
	manualset3
218549	9	420282	7	NULL	NULL	0	NULL	internal phase 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of several variables on nanoparticle characteristics was evaluated , including the ratio of drug-polymer , the amount of the poly vinyl alcohol as surfactant , and the internal phase volume/composition .
	manualset3
218550	10	420282	7	NULL	NULL	0	NULL	volume/composition	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of several variables on nanoparticle characteristics was evaluated , including the ratio of drug-polymer , the amount of the poly vinyl alcohol as surfactant , and the internal phase volume/composition .
	manualset3
218551	1	420283	7	NULL	NULL	0	NULL	small series	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this is a small series , a high rate of associated malignancy has been reported .
	manualset3
218552	2	420283	7	NULL	NULL	0	NULL	high rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this is a small series , a high rate of associated malignancy has been reported .
	manualset3
218553	3	420283	7	NULL	NULL	0	NULL	associated malignancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this is a small series , a high rate of associated malignancy has been reported .
	manualset3
218554	1	420284	7	NULL	NULL	0	NULL	 drug effects 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is not acceptable to use drug effects on plasma lipids or insulin resistance as measures of the effects on coronary heart disease , since dihydropyridine calcium antagonists improve these parameters while significantly increasing coronary heart disease events in the acute and chronic ischaemic situation .
	manualset3
218555	2	420284	7	NULL	NULL	0	NULL	 plasma lipids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is not acceptable to use drug effects on plasma lipids or insulin resistance as measures of the effects on coronary heart disease , since dihydropyridine calcium antagonists improve these parameters while significantly increasing coronary heart disease events in the acute and chronic ischaemic situation .
	manualset3
218556	3	420284	7	NULL	NULL	0	NULL	insulin resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is not acceptable to use drug effects on plasma lipids or insulin resistance as measures of the effects on coronary heart disease , since dihydropyridine calcium antagonists improve these parameters while significantly increasing coronary heart disease events in the acute and chronic ischaemic situation .
	manualset3
218557	4	420284	7	NULL	NULL	0	NULL	measures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is not acceptable to use drug effects on plasma lipids or insulin resistance as measures of the effects on coronary heart disease , since dihydropyridine calcium antagonists improve these parameters while significantly increasing coronary heart disease events in the acute and chronic ischaemic situation .
	manualset3
218558	5	420284	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is not acceptable to use drug effects on plasma lipids or insulin resistance as measures of the effects on coronary heart disease , since dihydropyridine calcium antagonists improve these parameters while significantly increasing coronary heart disease events in the acute and chronic ischaemic situation .
	manualset3
218559	6	420284	7	NULL	NULL	0	NULL	coronary heart disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It is not acceptable to use drug effects on plasma lipids or insulin resistance as measures of the effects on coronary heart disease , since dihydropyridine calcium antagonists improve these parameters while significantly increasing coronary heart disease events in the acute and chronic ischaemic situation .
	manualset3
218560	7	420284	7	NULL	NULL	0	NULL	 dihydropyridine calcium antagonists	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is not acceptable to use drug effects on plasma lipids or insulin resistance as measures of the effects on coronary heart disease , since dihydropyridine calcium antagonists improve these parameters while significantly increasing coronary heart disease events in the acute and chronic ischaemic situation .
	manualset3
218561	8	420284	7	NULL	NULL	0	NULL	parameters	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	It is not acceptable to use drug effects on plasma lipids or insulin resistance as measures of the effects on coronary heart disease , since dihydropyridine calcium antagonists improve these parameters while significantly increasing coronary heart disease events in the acute and chronic ischaemic situation .
	manualset3
218562	9	420284	7	NULL	NULL	0	NULL	coronary heart disease events	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is not acceptable to use drug effects on plasma lipids or insulin resistance as measures of the effects on coronary heart disease , since dihydropyridine calcium antagonists improve these parameters while significantly increasing coronary heart disease events in the acute and chronic ischaemic situation .
	manualset3
218563	10	420284	7	NULL	NULL	0	NULL	acute  ischaemic situation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is not acceptable to use drug effects on plasma lipids or insulin resistance as measures of the effects on coronary heart disease , since dihydropyridine calcium antagonists improve these parameters while significantly increasing coronary heart disease events in the acute and chronic ischaemic situation .
	manualset3
218564	11	420284	7	NULL	NULL	0	NULL	chronic ischaemic situation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is not acceptable to use drug effects on plasma lipids or insulin resistance as measures of the effects on coronary heart disease , since dihydropyridine calcium antagonists improve these parameters while significantly increasing coronary heart disease events in the acute and chronic ischaemic situation .
	manualset3
218565	1	420285	7	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We confirmed and further extended the number of cases with SMARCB1/INI1 inactivation to 6 of 11 cases , by real-time quantitative PCR analysis of mRNA expression and by SMARCB1/INI1 immunohistochemistry .
	manualset3
218566	2	420285	7	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We confirmed and further extended the number of cases with SMARCB1/INI1 inactivation to 6 of 11 cases , by real-time quantitative PCR analysis of mRNA expression and by SMARCB1/INI1 immunohistochemistry .
	manualset3
218567	3	420285	7	NULL	NULL	0	NULL	SMARCB1/INI1 inactivation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We confirmed and further extended the number of cases with SMARCB1/INI1 inactivation to 6 of 11 cases , by real-time quantitative PCR analysis of mRNA expression and by SMARCB1/INI1 immunohistochemistry .
	manualset3
218568	4	420285	7	NULL	NULL	0	NULL	6 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We confirmed and further extended the number of cases with SMARCB1/INI1 inactivation to 6 of 11 cases , by real-time quantitative PCR analysis of mRNA expression and by SMARCB1/INI1 immunohistochemistry .
	manualset3
218569	5	420285	7	NULL	NULL	0	NULL	11 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We confirmed and further extended the number of cases with SMARCB1/INI1 inactivation to 6 of 11 cases , by real-time quantitative PCR analysis of mRNA expression and by SMARCB1/INI1 immunohistochemistry .
	manualset3
218570	6	420285	7	NULL	NULL	0	NULL	real-time quantitative PCR analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We confirmed and further extended the number of cases with SMARCB1/INI1 inactivation to 6 of 11 cases , by real-time quantitative PCR analysis of mRNA expression and by SMARCB1/INI1 immunohistochemistry .
	manualset3
218571	7	420285	7	NULL	NULL	0	NULL	mRNA expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We confirmed and further extended the number of cases with SMARCB1/INI1 inactivation to 6 of 11 cases , by real-time quantitative PCR analysis of mRNA expression and by SMARCB1/INI1 immunohistochemistry .
	manualset3
218572	8	420285	7	NULL	NULL	0	NULL	SMARCB1/INI1 immunohistochemistry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We confirmed and further extended the number of cases with SMARCB1/INI1 inactivation to 6 of 11 cases , by real-time quantitative PCR analysis of mRNA expression and by SMARCB1/INI1 immunohistochemistry .
	manualset3
218573	1	420286	7	NULL	NULL	0	NULL	Unusual presentation	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Unusual presentation of a rhabdomyosarcoma of the ear .
	manualset3
218574	2	420286	7	NULL	NULL	0	NULL	rhabdomyosarcoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Unusual presentation of a rhabdomyosarcoma of the ear .
	manualset3
218575	3	420286	7	NULL	NULL	0	NULL	ear	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Unusual presentation of a rhabdomyosarcoma of the ear .
	manualset3
218576	1	420287	7	NULL	NULL	0	NULL	binding activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the binding activity of 11S15 'N was insensitive to GABA and 13N15 'S was stimulated much less than wildtype 13 by GABA .
	manualset3
218577	2	420287	7	NULL	NULL	0	NULL	11S15 'N	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the binding activity of 11S15 'N was insensitive to GABA and 13N15 'S was stimulated much less than wildtype 13 by GABA .
	manualset3
218578	3	420287	7	NULL	NULL	0	NULL	GABA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the binding activity of 11S15 'N was insensitive to GABA and 13N15 'S was stimulated much less than wildtype 13 by GABA .
	manualset3
218579	4	420287	7	NULL	NULL	0	NULL	13N15 'S	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the binding activity of 11S15 'N was insensitive to GABA and 13N15 'S was stimulated much less than wildtype 13 by GABA .
	manualset3
218580	5	420287	7	NULL	NULL	0	NULL	wildtype 13	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the binding activity of 11S15 'N was insensitive to GABA and 13N15 'S was stimulated much less than wildtype 13 by GABA .
	manualset3
218581	6	420287	7	NULL	NULL	0	NULL	GABA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the binding activity of 11S15 'N was insensitive to GABA and 13N15 'S was stimulated much less than wildtype 13 by GABA .
	manualset3
218582	1	420288	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results reported here may have implications concerning the structure of the opiate receptor complex and efforts to solubilize the binding protein in its native form .
	manualset3
218583	2	420288	7	NULL	NULL	0	NULL	implications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results reported here may have implications concerning the structure of the opiate receptor complex and efforts to solubilize the binding protein in its native form .
	manualset3
218584	3	420288	7	NULL	NULL	0	NULL	 structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results reported here may have implications concerning the structure of the opiate receptor complex and efforts to solubilize the binding protein in its native form .
	manualset3
218585	4	420288	7	NULL	NULL	0	NULL	opiate receptor complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results reported here may have implications concerning the structure of the opiate receptor complex and efforts to solubilize the binding protein in its native form .
	manualset3
218586	5	420288	7	NULL	NULL	0	NULL	binding protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results reported here may have implications concerning the structure of the opiate receptor complex and efforts to solubilize the binding protein in its native form .
	manualset3
218587	6	420288	7	NULL	NULL	0	NULL	native form	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The results reported here may have implications concerning the structure of the opiate receptor complex and efforts to solubilize the binding protein in its native form .
	manualset3
218588	1	420289	7	NULL	NULL	0	NULL	PFGE	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	PFGE and phage typing were also applied to study the role of direct transmission of E. coli O157 : H7 from cattle to humans on isolates collected from two separate farm outbreaks .
	manualset3
218589	2	420289	7	NULL	NULL	0	NULL	phage typing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	PFGE and phage typing were also applied to study the role of direct transmission of E. coli O157 : H7 from cattle to humans on isolates collected from two separate farm outbreaks .
	manualset3
218590	3	420289	7	NULL	NULL	0	NULL	role 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PFGE and phage typing were also applied to study the role of direct transmission of E. coli O157 : H7 from cattle to humans on isolates collected from two separate farm outbreaks .
	manualset3
218591	4	420289	7	NULL	NULL	0	NULL	direct transmission 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PFGE and phage typing were also applied to study the role of direct transmission of E. coli O157 : H7 from cattle to humans on isolates collected from two separate farm outbreaks .
	manualset3
218592	5	420289	7	NULL	NULL	0	NULL	E. coli O157 : H7	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	PFGE and phage typing were also applied to study the role of direct transmission of E. coli O157 : H7 from cattle to humans on isolates collected from two separate farm outbreaks .
	manualset3
218593	6	420289	7	NULL	NULL	0	NULL	cattle 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	PFGE and phage typing were also applied to study the role of direct transmission of E. coli O157 : H7 from cattle to humans on isolates collected from two separate farm outbreaks .
	manualset3
218594	7	420289	7	NULL	NULL	0	NULL	humans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	PFGE and phage typing were also applied to study the role of direct transmission of E. coli O157 : H7 from cattle to humans on isolates collected from two separate farm outbreaks .
	manualset3
218595	8	420289	7	NULL	NULL	NULL	NULL	two separate farm outbreaks	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	PFGE and phage typing were also applied to study the role of direct transmission of E. coli O157 : H7 from cattle to humans on isolates collected from two separate farm outbreaks .
	manualset3
219840	10	420289	7	NULL	NULL	0	NULL	isolates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	PFGE and phage typing were also applied to study the role of direct transmission of E. coli O157 : H7 from cattle to humans on isolates collected from two separate farm outbreaks .
	manualset3
218597	1	420290	7	NULL	NULL	0	NULL	Twenty-seven fractures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-seven fractures of the distal femur in 27 adult patients were treated with retrograde , interlocked , intramedullary nails after intercondylar fracture extension had been reduced and treated with lag screws .
	manualset3
218598	2	420290	7	NULL	NULL	0	NULL	 distal femur	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-seven fractures of the distal femur in 27 adult patients were treated with retrograde , interlocked , intramedullary nails after intercondylar fracture extension had been reduced and treated with lag screws .
	manualset3
218599	3	420290	7	NULL	NULL	0	NULL	27 adult patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-seven fractures of the distal femur in 27 adult patients were treated with retrograde , interlocked , intramedullary nails after intercondylar fracture extension had been reduced and treated with lag screws .
	manualset3
218600	4	420290	7	NULL	NULL	NULL	NULL	retrograde , interlocked , intramedullary nails	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Twenty-seven fractures of the distal femur in 27 adult patients were treated with retrograde , interlocked , intramedullary nails after intercondylar fracture extension had been reduced and treated with lag screws .
	manualset3
218601	5	420290	7	NULL	NULL	0	NULL	intercondylar fracture extension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-seven fractures of the distal femur in 27 adult patients were treated with retrograde , interlocked , intramedullary nails after intercondylar fracture extension had been reduced and treated with lag screws .
	manualset3
218602	6	420290	7	NULL	NULL	0	NULL	lag screws	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Twenty-seven fractures of the distal femur in 27 adult patients were treated with retrograde , interlocked , intramedullary nails after intercondylar fracture extension had been reduced and treated with lag screws .
	manualset3
218603	1	420291	7	NULL	NULL	0	NULL	Restoring	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Restoring the integrity of a disrupted biliary anastomosis can be difficult , and in some patients with that complication , neither the percutaneous technique nor the endoscopic approach effectively stents the biliary anastomosis .
	manualset3
218604	2	420291	7	NULL	NULL	0	NULL	integrity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Restoring the integrity of a disrupted biliary anastomosis can be difficult , and in some patients with that complication , neither the percutaneous technique nor the endoscopic approach effectively stents the biliary anastomosis .
	manualset3
218605	3	420291	7	NULL	NULL	0	NULL	disrupted biliary anastomosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Restoring the integrity of a disrupted biliary anastomosis can be difficult , and in some patients with that complication , neither the percutaneous technique nor the endoscopic approach effectively stents the biliary anastomosis .
	manualset3
218606	4	420291	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Restoring the integrity of a disrupted biliary anastomosis can be difficult , and in some patients with that complication , neither the percutaneous technique nor the endoscopic approach effectively stents the biliary anastomosis .
	manualset3
218607	5	420291	7	NULL	NULL	0	NULL	complication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Restoring the integrity of a disrupted biliary anastomosis can be difficult , and in some patients with that complication , neither the percutaneous technique nor the endoscopic approach effectively stents the biliary anastomosis .
	manualset3
218608	6	420291	7	NULL	NULL	0	NULL	percutaneous technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Restoring the integrity of a disrupted biliary anastomosis can be difficult , and in some patients with that complication , neither the percutaneous technique nor the endoscopic approach effectively stents the biliary anastomosis .
	manualset3
218609	7	420291	7	NULL	NULL	0	NULL	endoscopic approach 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Restoring the integrity of a disrupted biliary anastomosis can be difficult , and in some patients with that complication , neither the percutaneous technique nor the endoscopic approach effectively stents the biliary anastomosis .
	manualset3
218610	8	420291	7	NULL	NULL	0	NULL	biliary anastomosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Restoring the integrity of a disrupted biliary anastomosis can be difficult , and in some patients with that complication , neither the percutaneous technique nor the endoscopic approach effectively stents the biliary anastomosis .
	manualset3
218611	1	420292	7	NULL	NULL	0	NULL	 latter model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this latter model eventually resolves , it nonetheless represents inflammation in the clinically relevant setting of polymorphonuclear neutrophil/classically activated macrophage dominance driving a cytokine storm .
	manualset3
218612	2	420292	7	NULL	NULL	0	NULL	 inflammation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this latter model eventually resolves , it nonetheless represents inflammation in the clinically relevant setting of polymorphonuclear neutrophil/classically activated macrophage dominance driving a cytokine storm .
	manualset3
218613	3	420292	7	NULL	NULL	0	NULL	clinically relevant setting	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this latter model eventually resolves , it nonetheless represents inflammation in the clinically relevant setting of polymorphonuclear neutrophil/classically activated macrophage dominance driving a cytokine storm .
	manualset3
218614	4	420292	7	NULL	NULL	0	NULL	polymorphonuclear neutrophil	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this latter model eventually resolves , it nonetheless represents inflammation in the clinically relevant setting of polymorphonuclear neutrophil/classically activated macrophage dominance driving a cytokine storm .
	manualset3
218615	5	420292	7	NULL	NULL	0	NULL	classically activated macrophage dominance 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this latter model eventually resolves , it nonetheless represents inflammation in the clinically relevant setting of polymorphonuclear neutrophil/classically activated macrophage dominance driving a cytokine storm .
	manualset3
218616	6	420292	7	NULL	NULL	0	NULL	cytokine storm	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this latter model eventually resolves , it nonetheless represents inflammation in the clinically relevant setting of polymorphonuclear neutrophil/classically activated macrophage dominance driving a cytokine storm .
	manualset3
218617	1	420293	7	NULL	NULL	0	NULL	 westminster infirmary 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The westminster infirmary , 1872 .
	manualset3
218618	2	420293	7	NULL	NULL	0	NULL	1872	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The westminster infirmary , 1872 .
	manualset3
218619	1	420294	7	NULL	NULL	0	NULL	clues 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Further clues to the severity of MCA spasm were obtained from the ratio calculated dividing the MCA flow velocity by the flow velocity in the ipsilateral , extracranial internal carotid artery ( ICA ) , since spasm probably does not involve the neck vessels .
	manualset3
218620	2	420294	7	NULL	NULL	0	NULL	severity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Further clues to the severity of MCA spasm were obtained from the ratio calculated dividing the MCA flow velocity by the flow velocity in the ipsilateral , extracranial internal carotid artery ( ICA ) , since spasm probably does not involve the neck vessels .
	manualset3
218621	3	420294	7	NULL	NULL	0	NULL	MCA spasm	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Further clues to the severity of MCA spasm were obtained from the ratio calculated dividing the MCA flow velocity by the flow velocity in the ipsilateral , extracranial internal carotid artery ( ICA ) , since spasm probably does not involve the neck vessels .
	manualset3
218622	4	420294	7	NULL	NULL	0	NULL	ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Further clues to the severity of MCA spasm were obtained from the ratio calculated dividing the MCA flow velocity by the flow velocity in the ipsilateral , extracranial internal carotid artery ( ICA ) , since spasm probably does not involve the neck vessels .
	manualset3
218623	5	420294	7	NULL	NULL	0	NULL	MCA flow velocity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further clues to the severity of MCA spasm were obtained from the ratio calculated dividing the MCA flow velocity by the flow velocity in the ipsilateral , extracranial internal carotid artery ( ICA ) , since spasm probably does not involve the neck vessels .
	manualset3
218624	6	420294	7	NULL	NULL	0	NULL	flow velocity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further clues to the severity of MCA spasm were obtained from the ratio calculated dividing the MCA flow velocity by the flow velocity in the ipsilateral , extracranial internal carotid artery ( ICA ) , since spasm probably does not involve the neck vessels .
	manualset3
218625	7	420294	7	NULL	NULL	0	NULL	ipsilateral , extracranial internal carotid artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Further clues to the severity of MCA spasm were obtained from the ratio calculated dividing the MCA flow velocity by the flow velocity in the ipsilateral , extracranial internal carotid artery ( ICA ) , since spasm probably does not involve the neck vessels .
	manualset3
218626	8	420294	7	NULL	NULL	0	NULL	ICA	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Further clues to the severity of MCA spasm were obtained from the ratio calculated dividing the MCA flow velocity by the flow velocity in the ipsilateral , extracranial internal carotid artery ( ICA ) , since spasm probably does not involve the neck vessels .
	manualset3
218627	9	420294	7	NULL	NULL	0	NULL	 spasm 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Further clues to the severity of MCA spasm were obtained from the ratio calculated dividing the MCA flow velocity by the flow velocity in the ipsilateral , extracranial internal carotid artery ( ICA ) , since spasm probably does not involve the neck vessels .
	manualset3
218628	10	420294	7	NULL	NULL	0	NULL	neck vessels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Further clues to the severity of MCA spasm were obtained from the ratio calculated dividing the MCA flow velocity by the flow velocity in the ipsilateral , extracranial internal carotid artery ( ICA ) , since spasm probably does not involve the neck vessels .
	manualset3
218629	1	420295	7	NULL	NULL	0	NULL	PsADH1 isozymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The PsADH1 and PsADH2 isozymes appear to be equivalent in the ability to convert ethanol to acetaldehyde , and either is sufficient to allow cell growth on ethanol .
	manualset3
218630	2	420295	7	NULL	NULL	0	NULL	PsADH2 isozymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The PsADH1 and PsADH2 isozymes appear to be equivalent in the ability to convert ethanol to acetaldehyde , and either is sufficient to allow cell growth on ethanol .
	manualset3
218631	3	420295	7	NULL	NULL	0	NULL	ethanol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The PsADH1 and PsADH2 isozymes appear to be equivalent in the ability to convert ethanol to acetaldehyde , and either is sufficient to allow cell growth on ethanol .
	manualset3
218632	4	420295	7	NULL	NULL	0	NULL	acetaldehyde	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The PsADH1 and PsADH2 isozymes appear to be equivalent in the ability to convert ethanol to acetaldehyde , and either is sufficient to allow cell growth on ethanol .
	manualset3
218633	5	420295	7	NULL	NULL	0	NULL	cell growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The PsADH1 and PsADH2 isozymes appear to be equivalent in the ability to convert ethanol to acetaldehyde , and either is sufficient to allow cell growth on ethanol .
	manualset3
218634	6	420295	7	NULL	NULL	0	NULL	ethanol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The PsADH1 and PsADH2 isozymes appear to be equivalent in the ability to convert ethanol to acetaldehyde , and either is sufficient to allow cell growth on ethanol .
	manualset3
218635	7	420295	7	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The PsADH1 and PsADH2 isozymes appear to be equivalent in the ability to convert ethanol to acetaldehyde , and either is sufficient to allow cell growth on ethanol .
	manualset3
218636	1	420296	7	NULL	NULL	NULL	NULL	public educational campaigns	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Thus , public educational campaigns that focus on increasing awareness and knowledge about radon health risks and development of less expensive radon mitigation methods may help in promoting radon mitigation .
	manualset3
218637	2	420296	7	NULL	NULL	0	NULL	awareness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , public educational campaigns that focus on increasing awareness and knowledge about radon health risks and development of less expensive radon mitigation methods may help in promoting radon mitigation .
	manualset3
218638	3	420296	7	NULL	NULL	0	NULL	knowledge 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , public educational campaigns that focus on increasing awareness and knowledge about radon health risks and development of less expensive radon mitigation methods may help in promoting radon mitigation .
	manualset3
218639	4	420296	7	NULL	NULL	0	NULL	radon health risks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , public educational campaigns that focus on increasing awareness and knowledge about radon health risks and development of less expensive radon mitigation methods may help in promoting radon mitigation .
	manualset3
218640	5	420296	7	NULL	NULL	0	NULL	 development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , public educational campaigns that focus on increasing awareness and knowledge about radon health risks and development of less expensive radon mitigation methods may help in promoting radon mitigation .
	manualset3
218641	6	420296	7	NULL	NULL	0	NULL	radon mitigation methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , public educational campaigns that focus on increasing awareness and knowledge about radon health risks and development of less expensive radon mitigation methods may help in promoting radon mitigation .
	manualset3
218642	7	420296	7	NULL	NULL	0	NULL	radon mitigation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , public educational campaigns that focus on increasing awareness and knowledge about radon health risks and development of less expensive radon mitigation methods may help in promoting radon mitigation .
	manualset3
218643	1	420297	7	NULL	NULL	0	NULL	etiopathology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	After recalling the etiopathology of presbyacousis , the author analyzes the otological causes regarding the social isolation of the elderly .
	manualset3
218644	2	420297	7	NULL	NULL	0	NULL	presbyacousis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	After recalling the etiopathology of presbyacousis , the author analyzes the otological causes regarding the social isolation of the elderly .
	manualset3
218645	3	420297	7	NULL	NULL	0	NULL	author	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	After recalling the etiopathology of presbyacousis , the author analyzes the otological causes regarding the social isolation of the elderly .
	manualset3
218646	4	420297	7	NULL	NULL	0	NULL	otological causes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	After recalling the etiopathology of presbyacousis , the author analyzes the otological causes regarding the social isolation of the elderly .
	manualset3
218647	5	420297	7	NULL	NULL	0	NULL	social isolation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After recalling the etiopathology of presbyacousis , the author analyzes the otological causes regarding the social isolation of the elderly .
	manualset3
218648	6	420297	7	NULL	NULL	0	NULL	elderly	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	After recalling the etiopathology of presbyacousis , the author analyzes the otological causes regarding the social isolation of the elderly .
	manualset3
218649	1	420298	7	NULL	NULL	0	NULL	mAb	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this mAb has strong affinity/specificity for TEX101 , TES101 mAb loses its reactivity under reducing conditions .
	manualset3
218650	2	420298	7	NULL	NULL	0	NULL	affinity/specificity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this mAb has strong affinity/specificity for TEX101 , TES101 mAb loses its reactivity under reducing conditions .
	manualset3
218651	3	420298	7	NULL	NULL	0	NULL	 TEX101	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this mAb has strong affinity/specificity for TEX101 , TES101 mAb loses its reactivity under reducing conditions .
	manualset3
218652	4	420298	7	NULL	NULL	0	NULL	TES101 mAb	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this mAb has strong affinity/specificity for TEX101 , TES101 mAb loses its reactivity under reducing conditions .
	manualset3
218653	5	420298	7	NULL	NULL	0	NULL	reactivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this mAb has strong affinity/specificity for TEX101 , TES101 mAb loses its reactivity under reducing conditions .
	manualset3
218654	6	420298	7	NULL	NULL	0	NULL	 reducing conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this mAb has strong affinity/specificity for TEX101 , TES101 mAb loses its reactivity under reducing conditions .
	manualset3
218655	1	420299	7	NULL	NULL	0	NULL	in vitro model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	An in vitro model subjecting bladder muscle strips to continuous stretch relaxation evaluated-the properties of passive muscle length and tension .
	manualset3
218656	2	420299	7	NULL	NULL	0	NULL	bladder muscle strips	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An in vitro model subjecting bladder muscle strips to continuous stretch relaxation evaluated-the properties of passive muscle length and tension .
	manualset3
218657	3	420299	7	NULL	NULL	0	NULL	continuous stretch relaxation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An in vitro model subjecting bladder muscle strips to continuous stretch relaxation evaluated-the properties of passive muscle length and tension .
	manualset3
218658	4	420299	7	NULL	NULL	NULL	NULL	passive muscle length 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An in vitro model subjecting bladder muscle strips to continuous stretch relaxation evaluated-the properties of passive muscle length and tension .
	manualset3
218659	5	420299	7	NULL	NULL	NULL	NULL	tension	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An in vitro model subjecting bladder muscle strips to continuous stretch relaxation evaluated-the properties of passive muscle length and tension .
	manualset3
219841	6	420299	7	NULL	NULL	0	NULL	properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	An in vitro model subjecting bladder muscle strips to continuous stretch relaxation evaluated-the properties of passive muscle length and tension .
	manualset3
218660	1	420300	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results , complications , and technical aspects of occipital to posterior inferior cerebellar artery ( PICA ) bypass surgery are reviewed .
	manualset3
218661	2	420300	7	NULL	NULL	0	NULL	complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results , complications , and technical aspects of occipital to posterior inferior cerebellar artery ( PICA ) bypass surgery are reviewed .
	manualset3
218662	3	420300	7	NULL	NULL	0	NULL	technical aspects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results , complications , and technical aspects of occipital to posterior inferior cerebellar artery ( PICA ) bypass surgery are reviewed .
	manualset3
218663	4	420300	7	NULL	NULL	NULL	NULL	occipital 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results , complications , and technical aspects of occipital to posterior inferior cerebellar artery ( PICA ) bypass surgery are reviewed .
	manualset3
218664	6	420300	7	NULL	NULL	0	NULL	bypass surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results , complications , and technical aspects of occipital to posterior inferior cerebellar artery ( PICA ) bypass surgery are reviewed .
	manualset3
218665	5	420300	7	NULL	NULL	0	NULL	posterior inferior cerebellar artery ( PICA )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results , complications , and technical aspects of occipital to posterior inferior cerebellar artery ( PICA ) bypass surgery are reviewed .
	manualset3
218666	1	420301	7	NULL	NULL	0	NULL	Autophagy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Autophagy was evaluated by LC3-A protein expression .
	manualset3
218667	2	420301	7	NULL	NULL	0	NULL	LC3-A protein expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Autophagy was evaluated by LC3-A protein expression .
	manualset3
218668	1	420302	7	NULL	NULL	0	NULL	cut mandibular incisors	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cut mandibular incisors of group IV , the degree of the disturbance of odontogenesis and the atypical proliferation of odontogenic epithelium were more prominent ( p & lt ; 0.02 ) , and the dental lesions occurred earlier .
	manualset3
218669	2	420302	7	NULL	NULL	0	NULL	group IV	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cut mandibular incisors of group IV , the degree of the disturbance of odontogenesis and the atypical proliferation of odontogenic epithelium were more prominent ( p & lt ; 0.02 ) , and the dental lesions occurred earlier .
	manualset3
218670	3	420302	7	NULL	NULL	0	NULL	degree	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cut mandibular incisors of group IV , the degree of the disturbance of odontogenesis and the atypical proliferation of odontogenic epithelium were more prominent ( p & lt ; 0.02 ) , and the dental lesions occurred earlier .
	manualset3
218671	4	420302	7	NULL	NULL	0	NULL	disturbance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cut mandibular incisors of group IV , the degree of the disturbance of odontogenesis and the atypical proliferation of odontogenic epithelium were more prominent ( p & lt ; 0.02 ) , and the dental lesions occurred earlier .
	manualset3
218672	5	420302	7	NULL	NULL	0	NULL	odontogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cut mandibular incisors of group IV , the degree of the disturbance of odontogenesis and the atypical proliferation of odontogenic epithelium were more prominent ( p & lt ; 0.02 ) , and the dental lesions occurred earlier .
	manualset3
218673	6	420302	7	NULL	NULL	0	NULL	atypical proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cut mandibular incisors of group IV , the degree of the disturbance of odontogenesis and the atypical proliferation of odontogenic epithelium were more prominent ( p & lt ; 0.02 ) , and the dental lesions occurred earlier .
	manualset3
218674	7	420302	7	NULL	NULL	0	NULL	odontogenic epithelium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cut mandibular incisors of group IV , the degree of the disturbance of odontogenesis and the atypical proliferation of odontogenic epithelium were more prominent ( p & lt ; 0.02 ) , and the dental lesions occurred earlier .
	manualset3
218675	8	420302	7	NULL	NULL	0	NULL	p & lt ; 0.02	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cut mandibular incisors of group IV , the degree of the disturbance of odontogenesis and the atypical proliferation of odontogenic epithelium were more prominent ( p & lt ; 0.02 ) , and the dental lesions occurred earlier .
	manualset3
218676	9	420302	7	NULL	NULL	0	NULL	dental lesions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cut mandibular incisors of group IV , the degree of the disturbance of odontogenesis and the atypical proliferation of odontogenic epithelium were more prominent ( p & lt ; 0.02 ) , and the dental lesions occurred earlier .
	manualset3
218677	1	420303	7	NULL	NULL	NULL	NULL	average root mean squared deviation 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The average root mean squared deviation in the position for equivalent atoms between the 20 individual structures and the mean structure obtained by averaging their coordinates is 0.56 + / - 0.10 A for the main-chain atoms , and 0.95 + / - 0.09 A for all nonhydrogen atoms of residue 3 to 80 plus the heme group .
	manualset3
218678	2	420303	7	NULL	NULL	0	NULL	position	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The average root mean squared deviation in the position for equivalent atoms between the 20 individual structures and the mean structure obtained by averaging their coordinates is 0.56 + / - 0.10 A for the main-chain atoms , and 0.95 + / - 0.09 A for all nonhydrogen atoms of residue 3 to 80 plus the heme group .
	manualset3
218679	3	420303	7	NULL	NULL	0	NULL	equivalent atoms 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The average root mean squared deviation in the position for equivalent atoms between the 20 individual structures and the mean structure obtained by averaging their coordinates is 0.56 + / - 0.10 A for the main-chain atoms , and 0.95 + / - 0.09 A for all nonhydrogen atoms of residue 3 to 80 plus the heme group .
	manualset3
218680	4	420303	7	NULL	NULL	0	NULL	20 individual structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average root mean squared deviation in the position for equivalent atoms between the 20 individual structures and the mean structure obtained by averaging their coordinates is 0.56 + / - 0.10 A for the main-chain atoms , and 0.95 + / - 0.09 A for all nonhydrogen atoms of residue 3 to 80 plus the heme group .
	manualset3
218681	5	420303	7	NULL	NULL	0	NULL	mean structure 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average root mean squared deviation in the position for equivalent atoms between the 20 individual structures and the mean structure obtained by averaging their coordinates is 0.56 + / - 0.10 A for the main-chain atoms , and 0.95 + / - 0.09 A for all nonhydrogen atoms of residue 3 to 80 plus the heme group .
	manualset3
218682	6	420303	7	NULL	NULL	0	NULL	coordinates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average root mean squared deviation in the position for equivalent atoms between the 20 individual structures and the mean structure obtained by averaging their coordinates is 0.56 + / - 0.10 A for the main-chain atoms , and 0.95 + / - 0.09 A for all nonhydrogen atoms of residue 3 to 80 plus the heme group .
	manualset3
218683	7	420303	7	NULL	NULL	0	NULL	0.56 + / - 0.10 A	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average root mean squared deviation in the position for equivalent atoms between the 20 individual structures and the mean structure obtained by averaging their coordinates is 0.56 + / - 0.10 A for the main-chain atoms , and 0.95 + / - 0.09 A for all nonhydrogen atoms of residue 3 to 80 plus the heme group .
	manualset3
218684	8	420303	7	NULL	NULL	0	NULL	main-chain atoms	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The average root mean squared deviation in the position for equivalent atoms between the 20 individual structures and the mean structure obtained by averaging their coordinates is 0.56 + / - 0.10 A for the main-chain atoms , and 0.95 + / - 0.09 A for all nonhydrogen atoms of residue 3 to 80 plus the heme group .
	manualset3
218685	9	420303	7	NULL	NULL	0	NULL	0.95 + / - 0.09 A	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average root mean squared deviation in the position for equivalent atoms between the 20 individual structures and the mean structure obtained by averaging their coordinates is 0.56 + / - 0.10 A for the main-chain atoms , and 0.95 + / - 0.09 A for all nonhydrogen atoms of residue 3 to 80 plus the heme group .
	manualset3
218686	10	420303	7	NULL	NULL	0	NULL	nonhydrogen atoms	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	The average root mean squared deviation in the position for equivalent atoms between the 20 individual structures and the mean structure obtained by averaging their coordinates is 0.56 + / - 0.10 A for the main-chain atoms , and 0.95 + / - 0.09 A for all nonhydrogen atoms of residue 3 to 80 plus the heme group .
	manualset3
218687	11	420303	7	NULL	NULL	0	NULL	residue	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The average root mean squared deviation in the position for equivalent atoms between the 20 individual structures and the mean structure obtained by averaging their coordinates is 0.56 + / - 0.10 A for the main-chain atoms , and 0.95 + / - 0.09 A for all nonhydrogen atoms of residue 3 to 80 plus the heme group .
	manualset3
218688	12	420303	7	NULL	NULL	0	NULL	3 to 80	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The average root mean squared deviation in the position for equivalent atoms between the 20 individual structures and the mean structure obtained by averaging their coordinates is 0.56 + / - 0.10 A for the main-chain atoms , and 0.95 + / - 0.09 A for all nonhydrogen atoms of residue 3 to 80 plus the heme group .
	manualset3
218689	13	420303	7	NULL	NULL	0	NULL	heme group	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The average root mean squared deviation in the position for equivalent atoms between the 20 individual structures and the mean structure obtained by averaging their coordinates is 0.56 + / - 0.10 A for the main-chain atoms , and 0.95 + / - 0.09 A for all nonhydrogen atoms of residue 3 to 80 plus the heme group .
	manualset3
218690	1	420304	7	NULL	NULL	0	NULL	Extramammary Paget 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Extramammary Paget 's disease of the perineal skin : role of radiotherapy .
	manualset3
218691	2	420304	7	NULL	NULL	0	NULL	perineal skin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Extramammary Paget 's disease of the perineal skin : role of radiotherapy .
	manualset3
218692	3	420304	7	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Extramammary Paget 's disease of the perineal skin : role of radiotherapy .
	manualset3
218693	4	420304	7	NULL	NULL	0	NULL	radiotherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Extramammary Paget 's disease of the perineal skin : role of radiotherapy .
	manualset3
218694	1	420305	7	NULL	NULL	0	NULL	mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this mutation did not affect Jak1 association , stimulation-dependent phosphorylation of Jak1 was prevented .
	manualset3
218695	2	420305	7	NULL	NULL	0	NULL	Jak1 association	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this mutation did not affect Jak1 association , stimulation-dependent phosphorylation of Jak1 was prevented .
	manualset3
218696	3	420305	7	NULL	NULL	0	NULL	stimulation-dependent phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this mutation did not affect Jak1 association , stimulation-dependent phosphorylation of Jak1 was prevented .
	manualset3
218697	4	420305	7	NULL	NULL	0	NULL	Jak1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this mutation did not affect Jak1 association , stimulation-dependent phosphorylation of Jak1 was prevented .
	manualset3
218698	1	420306	7	NULL	NULL	0	NULL	direct injection method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the direct injection method , liquid-liquid extraction requires 1-2 ml of serum , plasma , or urine for clean-up .
	manualset3
218699	2	420306	7	NULL	NULL	0	NULL	liquid-liquid extraction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the direct injection method , liquid-liquid extraction requires 1-2 ml of serum , plasma , or urine for clean-up .
	manualset3
218700	3	420306	7	NULL	NULL	0	NULL	1-2 ml	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the direct injection method , liquid-liquid extraction requires 1-2 ml of serum , plasma , or urine for clean-up .
	manualset3
218701	4	420306	7	NULL	NULL	0	NULL	serum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the direct injection method , liquid-liquid extraction requires 1-2 ml of serum , plasma , or urine for clean-up .
	manualset3
218702	5	420306	7	NULL	NULL	0	NULL	plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the direct injection method , liquid-liquid extraction requires 1-2 ml of serum , plasma , or urine for clean-up .
	manualset3
218703	6	420306	7	NULL	NULL	0	NULL	urine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the direct injection method , liquid-liquid extraction requires 1-2 ml of serum , plasma , or urine for clean-up .
	manualset3
218704	7	420306	7	NULL	NULL	0	NULL	clean-up	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to the direct injection method , liquid-liquid extraction requires 1-2 ml of serum , plasma , or urine for clean-up .
	manualset3
218705	1	420307	7	NULL	NULL	0	NULL	medications	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , there is interest in whether medications used to treat depression alter the effects of nicotine .
	manualset3
218706	2	420307	7	NULL	NULL	0	NULL	depression	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , there is interest in whether medications used to treat depression alter the effects of nicotine .
	manualset3
218707	3	420307	7	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , there is interest in whether medications used to treat depression alter the effects of nicotine .
	manualset3
218708	4	420307	7	NULL	NULL	0	NULL	nicotine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , there is interest in whether medications used to treat depression alter the effects of nicotine .
	manualset3
218709	1	420308	7	NULL	NULL	0	NULL	gelsolin-like protein ( C/L-gelsolin ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We have previously identified a gelsolin-like protein ( C/L-gelsolin ) as a corneal crystallin in zebrafish .
	manualset3
218710	2	420308	7	NULL	NULL	0	NULL	 corneal crystallin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We have previously identified a gelsolin-like protein ( C/L-gelsolin ) as a corneal crystallin in zebrafish .
	manualset3
218711	3	420308	7	NULL	NULL	0	NULL	zebrafish	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We have previously identified a gelsolin-like protein ( C/L-gelsolin ) as a corneal crystallin in zebrafish .
	manualset3
218712	1	420309	7	NULL	NULL	0	NULL	travel plans	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , it demonstrates that travel plans can work , and are working , in the health sector .
	manualset3
218713	2	420309	7	NULL	NULL	0	NULL	health sector 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , it demonstrates that travel plans can work , and are working , in the health sector .
	manualset3
218714	3	420309	7	NULL	NULL	0	NULL	work	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , it demonstrates that travel plans can work , and are working , in the health sector .
	manualset3
218715	1	420310	7	NULL	NULL	0	NULL	Preclinical detection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Preclinical detection ( positron emission tomography and molecular genetics in some familial forms ) is a desirable goal with a view to neuroprotection .
	manualset3
218716	2	420310	7	NULL	NULL	0	NULL	positron emission tomography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Preclinical detection ( positron emission tomography and molecular genetics in some familial forms ) is a desirable goal with a view to neuroprotection .
	manualset3
218717	3	420310	7	NULL	NULL	0	NULL	molecular genetics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Preclinical detection ( positron emission tomography and molecular genetics in some familial forms ) is a desirable goal with a view to neuroprotection .
	manualset3
218718	4	420310	7	NULL	NULL	0	NULL	familial forms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Preclinical detection ( positron emission tomography and molecular genetics in some familial forms ) is a desirable goal with a view to neuroprotection .
	manualset3
218719	5	420310	7	NULL	NULL	0	NULL	desirable goal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Preclinical detection ( positron emission tomography and molecular genetics in some familial forms ) is a desirable goal with a view to neuroprotection .
	manualset3
218720	6	420310	7	NULL	NULL	NULL	NULL	 view	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Preclinical detection ( positron emission tomography and molecular genetics in some familial forms ) is a desirable goal with a view to neuroprotection .
	manualset3
218721	7	420310	7	NULL	NULL	0	NULL	neuroprotection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Preclinical detection ( positron emission tomography and molecular genetics in some familial forms ) is a desirable goal with a view to neuroprotection .
	manualset3
218722	1	420311	7	NULL	NULL	0	NULL	recent explosion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this recent explosion of innovation has brought advances to patient care , it has also brought concerns regarding overuse , increasing costs , and safety .
	manualset3
218723	2	420311	7	NULL	NULL	NULL	NULL	 innovation 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although this recent explosion of innovation has brought advances to patient care , it has also brought concerns regarding overuse , increasing costs , and safety .
	manualset3
218724	3	420311	7	NULL	NULL	0	NULL	patient care	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this recent explosion of innovation has brought advances to patient care , it has also brought concerns regarding overuse , increasing costs , and safety .
	manualset3
218725	4	420311	7	NULL	NULL	0	NULL	concerns	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this recent explosion of innovation has brought advances to patient care , it has also brought concerns regarding overuse , increasing costs , and safety .
	manualset3
218726	5	420311	7	NULL	NULL	0	NULL	overuse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this recent explosion of innovation has brought advances to patient care , it has also brought concerns regarding overuse , increasing costs , and safety .
	manualset3
218727	6	420311	7	NULL	NULL	0	NULL	 increasing costs 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this recent explosion of innovation has brought advances to patient care , it has also brought concerns regarding overuse , increasing costs , and safety .
	manualset3
218728	7	420311	7	NULL	NULL	0	NULL	safety	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this recent explosion of innovation has brought advances to patient care , it has also brought concerns regarding overuse , increasing costs , and safety .
	manualset3
218729	1	420312	7	NULL	NULL	0	NULL	tectal elements	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Second , these tectal elements have a local and global anatomical order across the tectum , which accounts for both the tripartite structure of the MURFs and their radial arrangement about a visual pole .
	manualset3
218730	2	420312	7	NULL	NULL	0	NULL	local anatomical order	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Second , these tectal elements have a local and global anatomical order across the tectum , which accounts for both the tripartite structure of the MURFs and their radial arrangement about a visual pole .
	manualset3
218731	3	420312	7	NULL	NULL	0	NULL	global anatomical order	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Second , these tectal elements have a local and global anatomical order across the tectum , which accounts for both the tripartite structure of the MURFs and their radial arrangement about a visual pole .
	manualset3
218732	4	420312	7	NULL	NULL	0	NULL	tectum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Second , these tectal elements have a local and global anatomical order across the tectum , which accounts for both the tripartite structure of the MURFs and their radial arrangement about a visual pole .
	manualset3
218733	5	420312	7	NULL	NULL	0	NULL	 tripartite structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Second , these tectal elements have a local and global anatomical order across the tectum , which accounts for both the tripartite structure of the MURFs and their radial arrangement about a visual pole .
	manualset3
218734	6	420312	7	NULL	NULL	0	NULL	MURFs	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Second , these tectal elements have a local and global anatomical order across the tectum , which accounts for both the tripartite structure of the MURFs and their radial arrangement about a visual pole .
	manualset3
218735	7	420312	7	NULL	NULL	0	NULL	radial arrangement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Second , these tectal elements have a local and global anatomical order across the tectum , which accounts for both the tripartite structure of the MURFs and their radial arrangement about a visual pole .
	manualset3
218736	8	420312	7	NULL	NULL	0	NULL	visual pole	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Second , these tectal elements have a local and global anatomical order across the tectum , which accounts for both the tripartite structure of the MURFs and their radial arrangement about a visual pole .
	manualset3
218737	1	420313	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the presence of interferon-gamma ( IFN - ) enhanced MSC capabilities to suppress T cell proliferation in vitro .
	manualset3
218738	2	420313	7	NULL	NULL	0	NULL	interferon-gamma ( IFN - ) enhanced MSC capabilities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the presence of interferon-gamma ( IFN - ) enhanced MSC capabilities to suppress T cell proliferation in vitro .
	manualset3
218739	3	420313	7	NULL	NULL	0	NULL	T cell proliferation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , the presence of interferon-gamma ( IFN - ) enhanced MSC capabilities to suppress T cell proliferation in vitro .
	manualset3
218740	1	420314	7	NULL	NULL	0	NULL	Down-regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Down-regulation of MoMLV mRNA occurred at the transcriptional level and was associated with decreased retrovirus production , as determined by titration experiments , suggesting that hypoxia may control MoMLV retroviral spread through the suppression of LTR activity .
	manualset3
218741	2	420314	7	NULL	NULL	0	NULL	MoMLV mRNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Down-regulation of MoMLV mRNA occurred at the transcriptional level and was associated with decreased retrovirus production , as determined by titration experiments , suggesting that hypoxia may control MoMLV retroviral spread through the suppression of LTR activity .
	manualset3
218742	3	420314	7	NULL	NULL	0	NULL	 transcriptional level 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Down-regulation of MoMLV mRNA occurred at the transcriptional level and was associated with decreased retrovirus production , as determined by titration experiments , suggesting that hypoxia may control MoMLV retroviral spread through the suppression of LTR activity .
	manualset3
218743	4	420314	7	NULL	NULL	0	NULL	decreased retrovirus production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Down-regulation of MoMLV mRNA occurred at the transcriptional level and was associated with decreased retrovirus production , as determined by titration experiments , suggesting that hypoxia may control MoMLV retroviral spread through the suppression of LTR activity .
	manualset3
218744	5	420314	7	NULL	NULL	0	NULL	titration experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Down-regulation of MoMLV mRNA occurred at the transcriptional level and was associated with decreased retrovirus production , as determined by titration experiments , suggesting that hypoxia may control MoMLV retroviral spread through the suppression of LTR activity .
	manualset3
218745	6	420314	7	NULL	NULL	0	NULL	hypoxia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Down-regulation of MoMLV mRNA occurred at the transcriptional level and was associated with decreased retrovirus production , as determined by titration experiments , suggesting that hypoxia may control MoMLV retroviral spread through the suppression of LTR activity .
	manualset3
218746	7	420314	7	NULL	NULL	0	NULL	MoMLV retroviral spread	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Down-regulation of MoMLV mRNA occurred at the transcriptional level and was associated with decreased retrovirus production , as determined by titration experiments , suggesting that hypoxia may control MoMLV retroviral spread through the suppression of LTR activity .
	manualset3
218747	8	420314	7	NULL	NULL	0	NULL	suppression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Down-regulation of MoMLV mRNA occurred at the transcriptional level and was associated with decreased retrovirus production , as determined by titration experiments , suggesting that hypoxia may control MoMLV retroviral spread through the suppression of LTR activity .
	manualset3
218748	9	420314	7	NULL	NULL	0	NULL	LTR activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Down-regulation of MoMLV mRNA occurred at the transcriptional level and was associated with decreased retrovirus production , as determined by titration experiments , suggesting that hypoxia may control MoMLV retroviral spread through the suppression of LTR activity .
	manualset3
218749	1	420315	7	NULL	NULL	0	NULL	variety	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Providing a variety of foods generally stimulates food intake and thereby might favor obesity .
	manualset3
218750	2	420315	7	NULL	NULL	0	NULL	 foods	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Providing a variety of foods generally stimulates food intake and thereby might favor obesity .
	manualset3
218751	3	420315	7	NULL	NULL	0	NULL	food intake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Providing a variety of foods generally stimulates food intake and thereby might favor obesity .
	manualset3
218752	4	420315	7	NULL	NULL	0	NULL	obesity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Providing a variety of foods generally stimulates food intake and thereby might favor obesity .
	manualset3
218753	1	420316	7	NULL	NULL	0	NULL	Correlations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlations in the partition thin-layer chromatography of alkali metals .
	manualset3
218754	2	420316	7	NULL	NULL	0	NULL	partition thin-layer chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlations in the partition thin-layer chromatography of alkali metals .
	manualset3
218755	3	420316	7	NULL	NULL	0	NULL	alkali metals 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlations in the partition thin-layer chromatography of alkali metals .
	manualset3
218756	1	420317	7	NULL	NULL	0	NULL	Chronic graft-versus-host disease ( cGVHD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic graft-versus-host disease ( cGVHD ) is a leading cause of allogeneic hematopoietic stem-cell transplantation-related mortality and morbidity .
	manualset3
218757	2	420317	7	NULL	NULL	0	NULL	leading cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic graft-versus-host disease ( cGVHD ) is a leading cause of allogeneic hematopoietic stem-cell transplantation-related mortality and morbidity .
	manualset3
218758	3	420317	7	NULL	NULL	0	NULL	allogeneic hematopoietic stem-cell transplantation-related mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic graft-versus-host disease ( cGVHD ) is a leading cause of allogeneic hematopoietic stem-cell transplantation-related mortality and morbidity .
	manualset3
218759	4	420317	7	NULL	NULL	0	NULL	morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic graft-versus-host disease ( cGVHD ) is a leading cause of allogeneic hematopoietic stem-cell transplantation-related mortality and morbidity .
	manualset3
218760	1	420318	7	NULL	NULL	0	NULL	9-week-old male	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In 9-week-old male anaesthetized LH rats and normotensive ( LL ) controls pretreated with an angiotensin-converting enzyme inhibitor ( quinapril ; 10 mg/kg ) and an AT1 receptor antagonist ( losartan ; 10 mg/kg ) , angiotensin ( Ang ) II was infused ( 30 ng/kg per min ) to stimulate AT2 receptors .
	manualset3
218761	2	420318	7	NULL	NULL	0	NULL	anaesthetized LH rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In 9-week-old male anaesthetized LH rats and normotensive ( LL ) controls pretreated with an angiotensin-converting enzyme inhibitor ( quinapril ; 10 mg/kg ) and an AT1 receptor antagonist ( losartan ; 10 mg/kg ) , angiotensin ( Ang ) II was infused ( 30 ng/kg per min ) to stimulate AT2 receptors .
	manualset3
218762	3	420318	7	NULL	NULL	0	NULL	normotensive ( LL ) controls	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 9-week-old male anaesthetized LH rats and normotensive ( LL ) controls pretreated with an angiotensin-converting enzyme inhibitor ( quinapril ; 10 mg/kg ) and an AT1 receptor antagonist ( losartan ; 10 mg/kg ) , angiotensin ( Ang ) II was infused ( 30 ng/kg per min ) to stimulate AT2 receptors .
	manualset3
218763	4	420318	7	NULL	NULL	0	NULL	angiotensin-converting enzyme inhibitor	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In 9-week-old male anaesthetized LH rats and normotensive ( LL ) controls pretreated with an angiotensin-converting enzyme inhibitor ( quinapril ; 10 mg/kg ) and an AT1 receptor antagonist ( losartan ; 10 mg/kg ) , angiotensin ( Ang ) II was infused ( 30 ng/kg per min ) to stimulate AT2 receptors .
	manualset3
218764	5	420318	7	NULL	NULL	0	NULL	quinapril	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In 9-week-old male anaesthetized LH rats and normotensive ( LL ) controls pretreated with an angiotensin-converting enzyme inhibitor ( quinapril ; 10 mg/kg ) and an AT1 receptor antagonist ( losartan ; 10 mg/kg ) , angiotensin ( Ang ) II was infused ( 30 ng/kg per min ) to stimulate AT2 receptors .
	manualset3
218765	6	420318	7	NULL	NULL	0	NULL	10 mg/kg 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 9-week-old male anaesthetized LH rats and normotensive ( LL ) controls pretreated with an angiotensin-converting enzyme inhibitor ( quinapril ; 10 mg/kg ) and an AT1 receptor antagonist ( losartan ; 10 mg/kg ) , angiotensin ( Ang ) II was infused ( 30 ng/kg per min ) to stimulate AT2 receptors .
	manualset3
218766	7	420318	7	NULL	NULL	0	NULL	AT1 receptor antagonist 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In 9-week-old male anaesthetized LH rats and normotensive ( LL ) controls pretreated with an angiotensin-converting enzyme inhibitor ( quinapril ; 10 mg/kg ) and an AT1 receptor antagonist ( losartan ; 10 mg/kg ) , angiotensin ( Ang ) II was infused ( 30 ng/kg per min ) to stimulate AT2 receptors .
	manualset3
218767	8	420318	7	NULL	NULL	0	NULL	losartan	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In 9-week-old male anaesthetized LH rats and normotensive ( LL ) controls pretreated with an angiotensin-converting enzyme inhibitor ( quinapril ; 10 mg/kg ) and an AT1 receptor antagonist ( losartan ; 10 mg/kg ) , angiotensin ( Ang ) II was infused ( 30 ng/kg per min ) to stimulate AT2 receptors .
	manualset3
218768	9	420318	7	NULL	NULL	0	NULL	10 mg/kg 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 9-week-old male anaesthetized LH rats and normotensive ( LL ) controls pretreated with an angiotensin-converting enzyme inhibitor ( quinapril ; 10 mg/kg ) and an AT1 receptor antagonist ( losartan ; 10 mg/kg ) , angiotensin ( Ang ) II was infused ( 30 ng/kg per min ) to stimulate AT2 receptors .
	manualset3
218769	10	420318	7	NULL	NULL	0	NULL	angiotensin ( Ang ) II 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In 9-week-old male anaesthetized LH rats and normotensive ( LL ) controls pretreated with an angiotensin-converting enzyme inhibitor ( quinapril ; 10 mg/kg ) and an AT1 receptor antagonist ( losartan ; 10 mg/kg ) , angiotensin ( Ang ) II was infused ( 30 ng/kg per min ) to stimulate AT2 receptors .
	manualset3
218770	11	420318	7	NULL	NULL	0	NULL	30 ng/kg per min	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 9-week-old male anaesthetized LH rats and normotensive ( LL ) controls pretreated with an angiotensin-converting enzyme inhibitor ( quinapril ; 10 mg/kg ) and an AT1 receptor antagonist ( losartan ; 10 mg/kg ) , angiotensin ( Ang ) II was infused ( 30 ng/kg per min ) to stimulate AT2 receptors .
	manualset3
218771	12	420318	7	NULL	NULL	0	NULL	AT2 receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In 9-week-old male anaesthetized LH rats and normotensive ( LL ) controls pretreated with an angiotensin-converting enzyme inhibitor ( quinapril ; 10 mg/kg ) and an AT1 receptor antagonist ( losartan ; 10 mg/kg ) , angiotensin ( Ang ) II was infused ( 30 ng/kg per min ) to stimulate AT2 receptors .
	manualset3
218772	1	420319	7	NULL	NULL	0	NULL	nephelometric determination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We have evaluated a nephelometric determination of serum haptoglobin .
	manualset3
218773	2	420319	7	NULL	NULL	0	NULL	serum haptoglobin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We have evaluated a nephelometric determination of serum haptoglobin .
	manualset3
218774	1	420320	7	NULL	NULL	0	NULL	Extravascular lung water volume ( EVLW )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Extravascular lung water volume ( EVLW ) , extravasation of 125I-serum albumin ( RISA ) into lung parenchyma , and albumin leak into the alveolar spaces were measured .
	manualset3
218775	2	420320	7	NULL	NULL	0	NULL	extravasation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Extravascular lung water volume ( EVLW ) , extravasation of 125I-serum albumin ( RISA ) into lung parenchyma , and albumin leak into the alveolar spaces were measured .
	manualset3
218776	3	420320	7	NULL	NULL	0	NULL	125I-serum albumin ( RISA )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Extravascular lung water volume ( EVLW ) , extravasation of 125I-serum albumin ( RISA ) into lung parenchyma , and albumin leak into the alveolar spaces were measured .
	manualset3
218777	4	420320	7	NULL	NULL	0	NULL	lung parenchyma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Extravascular lung water volume ( EVLW ) , extravasation of 125I-serum albumin ( RISA ) into lung parenchyma , and albumin leak into the alveolar spaces were measured .
	manualset3
218778	5	420320	7	NULL	NULL	0	NULL	albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Extravascular lung water volume ( EVLW ) , extravasation of 125I-serum albumin ( RISA ) into lung parenchyma , and albumin leak into the alveolar spaces were measured .
	manualset3
218779	6	420320	7	NULL	NULL	0	NULL	alveolar spaces	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Extravascular lung water volume ( EVLW ) , extravasation of 125I-serum albumin ( RISA ) into lung parenchyma , and albumin leak into the alveolar spaces were measured .
	manualset3
218780	1	420321	7	NULL	NULL	0	NULL	Experimental study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Experimental study on replica tooth implant ( author 's transl ) ) .
	manualset3
218781	2	420321	7	NULL	NULL	0	NULL	replica tooth implant	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Experimental study on replica tooth implant ( author 's transl ) ) .
	manualset3
218782	3	420321	7	NULL	NULL	0	NULL	author 's transl	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Experimental study on replica tooth implant ( author 's transl ) ) .
	manualset3
218783	1	420322	7	NULL	NULL	0	NULL	Ca2 + - dependent inositol phospholipid-specific phospholipase C activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It could be distinguished from the Ca2 + - dependent inositol phospholipid-specific phospholipase C activity in several rat tissues on the basis of its molecular size and its sensitivity to 1 , 10-phenanthroline .
	manualset3
218784	2	420322	7	NULL	NULL	0	NULL	several rat tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	It could be distinguished from the Ca2 + - dependent inositol phospholipid-specific phospholipase C activity in several rat tissues on the basis of its molecular size and its sensitivity to 1 , 10-phenanthroline .
	manualset3
218785	3	420322	7	NULL	NULL	0	NULL	basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It could be distinguished from the Ca2 + - dependent inositol phospholipid-specific phospholipase C activity in several rat tissues on the basis of its molecular size and its sensitivity to 1 , 10-phenanthroline .
	manualset3
218786	4	420322	7	NULL	NULL	0	NULL	molecular size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It could be distinguished from the Ca2 + - dependent inositol phospholipid-specific phospholipase C activity in several rat tissues on the basis of its molecular size and its sensitivity to 1 , 10-phenanthroline .
	manualset3
218787	5	420322	7	NULL	NULL	0	NULL	sensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It could be distinguished from the Ca2 + - dependent inositol phospholipid-specific phospholipase C activity in several rat tissues on the basis of its molecular size and its sensitivity to 1 , 10-phenanthroline .
	manualset3
218788	6	420322	7	NULL	NULL	0	NULL	1 , 10-phenanthroline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It could be distinguished from the Ca2 + - dependent inositol phospholipid-specific phospholipase C activity in several rat tissues on the basis of its molecular size and its sensitivity to 1 , 10-phenanthroline .
	manualset3
218789	1	420323	7	NULL	NULL	0	NULL	Different routes	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Different routes of progesterone administration and polycystic ovary syndrome : a review of the literature .
	manualset3
218790	2	420323	7	NULL	NULL	0	NULL	progesterone administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Different routes of progesterone administration and polycystic ovary syndrome : a review of the literature .
	manualset3
218791	3	420323	7	NULL	NULL	0	NULL	polycystic ovary syndrome 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Different routes of progesterone administration and polycystic ovary syndrome : a review of the literature .
	manualset3
218792	4	420323	7	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Different routes of progesterone administration and polycystic ovary syndrome : a review of the literature .
	manualset3
218793	5	420323	7	NULL	NULL	0	NULL	literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Different routes of progesterone administration and polycystic ovary syndrome : a review of the literature .
	manualset3
218794	1	420324	7	NULL	NULL	0	NULL	specimens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The specimens revealed multicentric , bilateral C-cell carcinomas .
	manualset3
218795	2	420324	7	NULL	NULL	0	NULL	multicentric  C-cell carcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The specimens revealed multicentric , bilateral C-cell carcinomas .
	manualset3
218796	3	420324	7	NULL	NULL	0	NULL	bilateral C-cell carcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The specimens revealed multicentric , bilateral C-cell carcinomas .
	manualset3
218797	1	420325	7	NULL	NULL	0	NULL	purification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purification and specificity of a lipase fromVernonia anthelmintica seed .
	manualset3
218798	2	420325	7	NULL	NULL	0	NULL	specificity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purification and specificity of a lipase fromVernonia anthelmintica seed .
	manualset3
218799	3	420325	7	NULL	NULL	0	NULL	lipase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The purification and specificity of a lipase fromVernonia anthelmintica seed .
	manualset3
218800	4	420325	7	NULL	NULL	0	NULL	Vernonia anthelmintica seed	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The purification and specificity of a lipase fromVernonia anthelmintica seed .
	manualset3
218801	1	420326	7	NULL	NULL	0	NULL	first period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Except for the first period , the allograft LPO and GSH-Px levels rose for up to 6 years after transplantation .
	manualset3
218802	2	420326	7	NULL	NULL	0	NULL	allograft LPO levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Except for the first period , the allograft LPO and GSH-Px levels rose for up to 6 years after transplantation .
	manualset3
218803	3	420326	7	NULL	NULL	0	NULL	GSH-Px levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Except for the first period , the allograft LPO and GSH-Px levels rose for up to 6 years after transplantation .
	manualset3
218804	4	420326	7	NULL	NULL	0	NULL	 6 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Except for the first period , the allograft LPO and GSH-Px levels rose for up to 6 years after transplantation .
	manualset3
218805	5	420326	7	NULL	NULL	0	NULL	transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Except for the first period , the allograft LPO and GSH-Px levels rose for up to 6 years after transplantation .
	manualset3
218806	1	420327	7	NULL	NULL	0	NULL	microprocessor	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Several microprocessor exercise physiology systems have been introduced recently .
	manualset3
218807	2	420327	7	NULL	NULL	0	NULL	physiology systems	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Several microprocessor exercise physiology systems have been introduced recently .
	manualset3
218808	1	420328	7	NULL	NULL	0	NULL	variant streptococcus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this variant streptococcus grew aerobically on chocolate agar , the isolate would not grow on blood agar , the medium used to screen for S. pyogenes , unless it was incubated anaerobically or incubated in air with cocarboxylase .
	manualset3
218809	2	420328	7	NULL	NULL	NULL	NULL	 chocolate agar	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although this variant streptococcus grew aerobically on chocolate agar , the isolate would not grow on blood agar , the medium used to screen for S. pyogenes , unless it was incubated anaerobically or incubated in air with cocarboxylase .
	manualset3
218810	3	420328	7	NULL	NULL	0	NULL	isolate	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this variant streptococcus grew aerobically on chocolate agar , the isolate would not grow on blood agar , the medium used to screen for S. pyogenes , unless it was incubated anaerobically or incubated in air with cocarboxylase .
	manualset3
218811	4	420328	7	NULL	NULL	0	NULL	blood agar	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this variant streptococcus grew aerobically on chocolate agar , the isolate would not grow on blood agar , the medium used to screen for S. pyogenes , unless it was incubated anaerobically or incubated in air with cocarboxylase .
	manualset3
218812	5	420328	7	NULL	NULL	0	NULL	medium	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this variant streptococcus grew aerobically on chocolate agar , the isolate would not grow on blood agar , the medium used to screen for S. pyogenes , unless it was incubated anaerobically or incubated in air with cocarboxylase .
	manualset3
218813	6	420328	7	NULL	NULL	0	NULL	S. pyogenes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this variant streptococcus grew aerobically on chocolate agar , the isolate would not grow on blood agar , the medium used to screen for S. pyogenes , unless it was incubated anaerobically or incubated in air with cocarboxylase .
	manualset3
218814	7	420328	7	NULL	NULL	0	NULL	air	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this variant streptococcus grew aerobically on chocolate agar , the isolate would not grow on blood agar , the medium used to screen for S. pyogenes , unless it was incubated anaerobically or incubated in air with cocarboxylase .
	manualset3
218815	8	420328	7	NULL	NULL	0	NULL	cocarboxylase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although this variant streptococcus grew aerobically on chocolate agar , the isolate would not grow on blood agar , the medium used to screen for S. pyogenes , unless it was incubated anaerobically or incubated in air with cocarboxylase .
	manualset3
218816	1	420329	7	NULL	NULL	0	NULL	Azithromycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Azithromycin and erythromycin disk test results were compared to MIC values obtained in six different media .
	manualset3
218817	2	420329	7	NULL	NULL	0	NULL	erythromycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Azithromycin and erythromycin disk test results were compared to MIC values obtained in six different media .
	manualset3
218818	3	420329	7	NULL	NULL	0	NULL	disk test results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Azithromycin and erythromycin disk test results were compared to MIC values obtained in six different media .
	manualset3
218819	4	420329	7	NULL	NULL	0	NULL	MIC values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Azithromycin and erythromycin disk test results were compared to MIC values obtained in six different media .
	manualset3
218820	5	420329	7	NULL	NULL	0	NULL	six different media 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Azithromycin and erythromycin disk test results were compared to MIC values obtained in six different media .
	manualset3
218821	1	420330	7	NULL	NULL	0	NULL	gene ( nonR )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A gene ( nonR ) conferring tetranactin resistance on the macrotetrolide-sensitive strain , Streptomyces lividans TK64 , was isolated during a shotgun cloning experiment , in which chromosomal fragments from Streptomyces griseus were ligated into the vector pIJ699 and then introduced by transformation into S. lividans TK64 .
	manualset3
218822	2	420330	7	NULL	NULL	0	NULL	tetranactin resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A gene ( nonR ) conferring tetranactin resistance on the macrotetrolide-sensitive strain , Streptomyces lividans TK64 , was isolated during a shotgun cloning experiment , in which chromosomal fragments from Streptomyces griseus were ligated into the vector pIJ699 and then introduced by transformation into S. lividans TK64 .
	manualset3
218823	3	420330	7	NULL	NULL	0	NULL	macrotetrolide-sensitive strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A gene ( nonR ) conferring tetranactin resistance on the macrotetrolide-sensitive strain , Streptomyces lividans TK64 , was isolated during a shotgun cloning experiment , in which chromosomal fragments from Streptomyces griseus were ligated into the vector pIJ699 and then introduced by transformation into S. lividans TK64 .
	manualset3
218824	4	420330	7	NULL	NULL	0	NULL	Streptomyces lividans TK64	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A gene ( nonR ) conferring tetranactin resistance on the macrotetrolide-sensitive strain , Streptomyces lividans TK64 , was isolated during a shotgun cloning experiment , in which chromosomal fragments from Streptomyces griseus were ligated into the vector pIJ699 and then introduced by transformation into S. lividans TK64 .
	manualset3
218825	5	420330	7	NULL	NULL	0	NULL	shotgun cloning experiment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A gene ( nonR ) conferring tetranactin resistance on the macrotetrolide-sensitive strain , Streptomyces lividans TK64 , was isolated during a shotgun cloning experiment , in which chromosomal fragments from Streptomyces griseus were ligated into the vector pIJ699 and then introduced by transformation into S. lividans TK64 .
	manualset3
218826	6	420330	7	NULL	NULL	0	NULL	chromosomal fragments	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	A gene ( nonR ) conferring tetranactin resistance on the macrotetrolide-sensitive strain , Streptomyces lividans TK64 , was isolated during a shotgun cloning experiment , in which chromosomal fragments from Streptomyces griseus were ligated into the vector pIJ699 and then introduced by transformation into S. lividans TK64 .
	manualset3
218827	7	420330	7	NULL	NULL	0	NULL	Streptomyces griseus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A gene ( nonR ) conferring tetranactin resistance on the macrotetrolide-sensitive strain , Streptomyces lividans TK64 , was isolated during a shotgun cloning experiment , in which chromosomal fragments from Streptomyces griseus were ligated into the vector pIJ699 and then introduced by transformation into S. lividans TK64 .
	manualset3
218828	8	420330	7	NULL	NULL	0	NULL	vector pIJ699	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A gene ( nonR ) conferring tetranactin resistance on the macrotetrolide-sensitive strain , Streptomyces lividans TK64 , was isolated during a shotgun cloning experiment , in which chromosomal fragments from Streptomyces griseus were ligated into the vector pIJ699 and then introduced by transformation into S. lividans TK64 .
	manualset3
218829	9	420330	7	NULL	NULL	0	NULL	transformation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A gene ( nonR ) conferring tetranactin resistance on the macrotetrolide-sensitive strain , Streptomyces lividans TK64 , was isolated during a shotgun cloning experiment , in which chromosomal fragments from Streptomyces griseus were ligated into the vector pIJ699 and then introduced by transformation into S. lividans TK64 .
	manualset3
218830	10	420330	7	NULL	NULL	0	NULL	S. lividans TK64	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A gene ( nonR ) conferring tetranactin resistance on the macrotetrolide-sensitive strain , Streptomyces lividans TK64 , was isolated during a shotgun cloning experiment , in which chromosomal fragments from Streptomyces griseus were ligated into the vector pIJ699 and then introduced by transformation into S. lividans TK64 .
	manualset3
218913	1	420331	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that suicide attempts do not constitute a very large problem in children aged 5-14 ; attempts hardly occur at all in children under the age of 11 , but the incidence increases with age .
	manualset3
218914	2	420331	7	NULL	NULL	0	NULL	 suicide attempts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that suicide attempts do not constitute a very large problem in children aged 5-14 ; attempts hardly occur at all in children under the age of 11 , but the incidence increases with age .
	manualset3
218915	3	420331	7	NULL	NULL	0	NULL	large problem	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that suicide attempts do not constitute a very large problem in children aged 5-14 ; attempts hardly occur at all in children under the age of 11 , but the incidence increases with age .
	manualset3
218916	4	420331	7	NULL	NULL	0	NULL	 children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that suicide attempts do not constitute a very large problem in children aged 5-14 ; attempts hardly occur at all in children under the age of 11 , but the incidence increases with age .
	manualset3
218917	5	420331	7	NULL	NULL	0	NULL	 5-14	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that suicide attempts do not constitute a very large problem in children aged 5-14 ; attempts hardly occur at all in children under the age of 11 , but the incidence increases with age .
	manualset3
218918	6	420331	7	NULL	NULL	0	NULL	attempts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that suicide attempts do not constitute a very large problem in children aged 5-14 ; attempts hardly occur at all in children under the age of 11 , but the incidence increases with age .
	manualset3
218919	7	420331	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that suicide attempts do not constitute a very large problem in children aged 5-14 ; attempts hardly occur at all in children under the age of 11 , but the incidence increases with age .
	manualset3
218920	8	420331	7	NULL	NULL	0	NULL	age 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that suicide attempts do not constitute a very large problem in children aged 5-14 ; attempts hardly occur at all in children under the age of 11 , but the incidence increases with age .
	manualset3
218921	9	420331	7	NULL	NULL	0	NULL	 11	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that suicide attempts do not constitute a very large problem in children aged 5-14 ; attempts hardly occur at all in children under the age of 11 , but the incidence increases with age .
	manualset3
218922	10	420331	7	NULL	NULL	0	NULL	 incidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that suicide attempts do not constitute a very large problem in children aged 5-14 ; attempts hardly occur at all in children under the age of 11 , but the incidence increases with age .
	manualset3
218923	11	420331	7	NULL	NULL	0	NULL	age	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that suicide attempts do not constitute a very large problem in children aged 5-14 ; attempts hardly occur at all in children under the age of 11 , but the incidence increases with age .
	manualset3
218924	1	420332	7	NULL	NULL	0	NULL	 similar changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that similar changes may take place in the human myocardium and may underlie the cardiac weakness .
	manualset3
218925	2	420332	7	NULL	NULL	0	NULL	human myocardium 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that similar changes may take place in the human myocardium and may underlie the cardiac weakness .
	manualset3
218926	3	420332	7	NULL	NULL	0	NULL	cardiac weakness 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	It is suggested that similar changes may take place in the human myocardium and may underlie the cardiac weakness .
	manualset3
218927	1	420333	7	NULL	NULL	0	NULL	15 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 15 patients with the normal body mass and disturbed glucose tolerance a glycemia level was higher and insulin levels lower than in 10 healthy persons in the first 20 min after i. v. insulin injection ( 1.2 units per 1 m2 of the body surface ) .
	manualset3
218928	2	420333	7	NULL	NULL	0	NULL	normal body mass	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 15 patients with the normal body mass and disturbed glucose tolerance a glycemia level was higher and insulin levels lower than in 10 healthy persons in the first 20 min after i. v. insulin injection ( 1.2 units per 1 m2 of the body surface ) .
	manualset3
218929	3	420333	7	NULL	NULL	NULL	NULL	disturbed glucose tolerance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In 15 patients with the normal body mass and disturbed glucose tolerance a glycemia level was higher and insulin levels lower than in 10 healthy persons in the first 20 min after i. v. insulin injection ( 1.2 units per 1 m2 of the body surface ) .
	manualset3
218930	4	420333	7	NULL	NULL	0	NULL	glycemia level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 15 patients with the normal body mass and disturbed glucose tolerance a glycemia level was higher and insulin levels lower than in 10 healthy persons in the first 20 min after i. v. insulin injection ( 1.2 units per 1 m2 of the body surface ) .
	manualset3
218931	5	420333	7	NULL	NULL	0	NULL	insulin levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 15 patients with the normal body mass and disturbed glucose tolerance a glycemia level was higher and insulin levels lower than in 10 healthy persons in the first 20 min after i. v. insulin injection ( 1.2 units per 1 m2 of the body surface ) .
	manualset3
218932	6	420333	7	NULL	NULL	0	NULL	10 healthy persons	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 15 patients with the normal body mass and disturbed glucose tolerance a glycemia level was higher and insulin levels lower than in 10 healthy persons in the first 20 min after i. v. insulin injection ( 1.2 units per 1 m2 of the body surface ) .
	manualset3
218933	7	420333	7	NULL	NULL	0	NULL	first 20 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In 15 patients with the normal body mass and disturbed glucose tolerance a glycemia level was higher and insulin levels lower than in 10 healthy persons in the first 20 min after i. v. insulin injection ( 1.2 units per 1 m2 of the body surface ) .
	manualset3
218934	8	420333	7	NULL	NULL	0	NULL	 i. v. insulin injection	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In 15 patients with the normal body mass and disturbed glucose tolerance a glycemia level was higher and insulin levels lower than in 10 healthy persons in the first 20 min after i. v. insulin injection ( 1.2 units per 1 m2 of the body surface ) .
	manualset3
218935	9	420333	7	NULL	NULL	0	NULL	1.2 units per 1 m2	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 15 patients with the normal body mass and disturbed glucose tolerance a glycemia level was higher and insulin levels lower than in 10 healthy persons in the first 20 min after i. v. insulin injection ( 1.2 units per 1 m2 of the body surface ) .
	manualset3
218936	10	420333	7	NULL	NULL	0	NULL	body surface	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In 15 patients with the normal body mass and disturbed glucose tolerance a glycemia level was higher and insulin levels lower than in 10 healthy persons in the first 20 min after i. v. insulin injection ( 1.2 units per 1 m2 of the body surface ) .
	manualset3
218937	1	420334	7	NULL	NULL	0	NULL	Decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Decrease in lipopolysaccharide ( LPS ) - induced proliferation of the peripheral blood mononuclear cells ( PBMCs ) , one of the functional readouts of the innate immune system , has also been observed in frail older adults .
	manualset3
218938	2	420334	7	NULL	NULL	0	NULL	lipopolysaccharide ( LPS ) - induced proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Decrease in lipopolysaccharide ( LPS ) - induced proliferation of the peripheral blood mononuclear cells ( PBMCs ) , one of the functional readouts of the innate immune system , has also been observed in frail older adults .
	manualset3
218939	3	420334	7	NULL	NULL	0	NULL	peripheral blood mononuclear cells ( PBMCs )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Decrease in lipopolysaccharide ( LPS ) - induced proliferation of the peripheral blood mononuclear cells ( PBMCs ) , one of the functional readouts of the innate immune system , has also been observed in frail older adults .
	manualset3
218940	4	420334	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Decrease in lipopolysaccharide ( LPS ) - induced proliferation of the peripheral blood mononuclear cells ( PBMCs ) , one of the functional readouts of the innate immune system , has also been observed in frail older adults .
	manualset3
218941	5	420334	7	NULL	NULL	0	NULL	functional readouts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Decrease in lipopolysaccharide ( LPS ) - induced proliferation of the peripheral blood mononuclear cells ( PBMCs ) , one of the functional readouts of the innate immune system , has also been observed in frail older adults .
	manualset3
218942	6	420334	7	NULL	NULL	0	NULL	innate immune system 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Decrease in lipopolysaccharide ( LPS ) - induced proliferation of the peripheral blood mononuclear cells ( PBMCs ) , one of the functional readouts of the innate immune system , has also been observed in frail older adults .
	manualset3
218943	7	420334	7	NULL	NULL	0	NULL	frail older adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Decrease in lipopolysaccharide ( LPS ) - induced proliferation of the peripheral blood mononuclear cells ( PBMCs ) , one of the functional readouts of the innate immune system , has also been observed in frail older adults .
	manualset3
218944	1	420335	7	NULL	NULL	0	NULL	strongest antibacterial effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The strongest antibacterial effect at 24 hours was shown by a `` soft '' mix of IRM .
	manualset3
218945	2	420335	7	NULL	NULL	0	NULL	24 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The strongest antibacterial effect at 24 hours was shown by a `` soft '' mix of IRM .
	manualset3
218946	3	420335	7	NULL	NULL	0	NULL	 `` soft '' mix	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The strongest antibacterial effect at 24 hours was shown by a `` soft '' mix of IRM .
	manualset3
218947	4	420335	7	NULL	NULL	0	NULL	IRM	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The strongest antibacterial effect at 24 hours was shown by a `` soft '' mix of IRM .
	manualset3
218948	1	420336	7	NULL	NULL	0	NULL	Investigation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation revealed minimal change glomerulonephritis and non-Hodgkins lymphoma .
	manualset3
218949	2	420336	7	NULL	NULL	0	NULL	minimal change glomerulonephritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation revealed minimal change glomerulonephritis and non-Hodgkins lymphoma .
	manualset3
218950	3	420336	7	NULL	NULL	0	NULL	non-Hodgkins lymphoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation revealed minimal change glomerulonephritis and non-Hodgkins lymphoma .
	manualset3
218951	1	420337	7	NULL	NULL	0	NULL	further studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although further studies are necessary to corroborate and assess the overall incidence of these polymorphisms in human populations , the use of W-CGH could be pertinent and of clinical relevance to assess rapidly , from a chromosomal viewpoint , genome similarities and differences in closely related genomes such as those of relatives , or in more specific situations such as bone marrow transplantation where chimerism is produced in the recipient .
	manualset3
218952	2	420337	7	NULL	NULL	0	NULL	overall incidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although further studies are necessary to corroborate and assess the overall incidence of these polymorphisms in human populations , the use of W-CGH could be pertinent and of clinical relevance to assess rapidly , from a chromosomal viewpoint , genome similarities and differences in closely related genomes such as those of relatives , or in more specific situations such as bone marrow transplantation where chimerism is produced in the recipient .
	manualset3
218953	3	420337	7	NULL	NULL	0	NULL	polymorphisms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although further studies are necessary to corroborate and assess the overall incidence of these polymorphisms in human populations , the use of W-CGH could be pertinent and of clinical relevance to assess rapidly , from a chromosomal viewpoint , genome similarities and differences in closely related genomes such as those of relatives , or in more specific situations such as bone marrow transplantation where chimerism is produced in the recipient .
	manualset3
218954	4	420337	7	NULL	NULL	0	NULL	human populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although further studies are necessary to corroborate and assess the overall incidence of these polymorphisms in human populations , the use of W-CGH could be pertinent and of clinical relevance to assess rapidly , from a chromosomal viewpoint , genome similarities and differences in closely related genomes such as those of relatives , or in more specific situations such as bone marrow transplantation where chimerism is produced in the recipient .
	manualset3
218955	5	420337	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although further studies are necessary to corroborate and assess the overall incidence of these polymorphisms in human populations , the use of W-CGH could be pertinent and of clinical relevance to assess rapidly , from a chromosomal viewpoint , genome similarities and differences in closely related genomes such as those of relatives , or in more specific situations such as bone marrow transplantation where chimerism is produced in the recipient .
	manualset3
218956	6	420337	7	NULL	NULL	0	NULL	W-CGH	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although further studies are necessary to corroborate and assess the overall incidence of these polymorphisms in human populations , the use of W-CGH could be pertinent and of clinical relevance to assess rapidly , from a chromosomal viewpoint , genome similarities and differences in closely related genomes such as those of relatives , or in more specific situations such as bone marrow transplantation where chimerism is produced in the recipient .
	manualset3
218957	7	420337	7	NULL	NULL	0	NULL	clinical relevance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although further studies are necessary to corroborate and assess the overall incidence of these polymorphisms in human populations , the use of W-CGH could be pertinent and of clinical relevance to assess rapidly , from a chromosomal viewpoint , genome similarities and differences in closely related genomes such as those of relatives , or in more specific situations such as bone marrow transplantation where chimerism is produced in the recipient .
	manualset3
218958	8	420337	7	NULL	NULL	0	NULL	chromosomal viewpoint	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although further studies are necessary to corroborate and assess the overall incidence of these polymorphisms in human populations , the use of W-CGH could be pertinent and of clinical relevance to assess rapidly , from a chromosomal viewpoint , genome similarities and differences in closely related genomes such as those of relatives , or in more specific situations such as bone marrow transplantation where chimerism is produced in the recipient .
	manualset3
218959	9	420337	7	NULL	NULL	0	NULL	genome similarities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although further studies are necessary to corroborate and assess the overall incidence of these polymorphisms in human populations , the use of W-CGH could be pertinent and of clinical relevance to assess rapidly , from a chromosomal viewpoint , genome similarities and differences in closely related genomes such as those of relatives , or in more specific situations such as bone marrow transplantation where chimerism is produced in the recipient .
	manualset3
218960	10	420337	7	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Although further studies are necessary to corroborate and assess the overall incidence of these polymorphisms in human populations , the use of W-CGH could be pertinent and of clinical relevance to assess rapidly , from a chromosomal viewpoint , genome similarities and differences in closely related genomes such as those of relatives , or in more specific situations such as bone marrow transplantation where chimerism is produced in the recipient .
	manualset3
218961	11	420337	7	NULL	NULL	0	NULL	closely related genomes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Although further studies are necessary to corroborate and assess the overall incidence of these polymorphisms in human populations , the use of W-CGH could be pertinent and of clinical relevance to assess rapidly , from a chromosomal viewpoint , genome similarities and differences in closely related genomes such as those of relatives , or in more specific situations such as bone marrow transplantation where chimerism is produced in the recipient .
	manualset3
218962	12	420337	7	NULL	NULL	0	NULL	 relatives	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Although further studies are necessary to corroborate and assess the overall incidence of these polymorphisms in human populations , the use of W-CGH could be pertinent and of clinical relevance to assess rapidly , from a chromosomal viewpoint , genome similarities and differences in closely related genomes such as those of relatives , or in more specific situations such as bone marrow transplantation where chimerism is produced in the recipient .
	manualset3
218963	13	420337	7	NULL	NULL	0	NULL	specific situations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although further studies are necessary to corroborate and assess the overall incidence of these polymorphisms in human populations , the use of W-CGH could be pertinent and of clinical relevance to assess rapidly , from a chromosomal viewpoint , genome similarities and differences in closely related genomes such as those of relatives , or in more specific situations such as bone marrow transplantation where chimerism is produced in the recipient .
	manualset3
218964	14	420337	7	NULL	NULL	0	NULL	bone marrow transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Although further studies are necessary to corroborate and assess the overall incidence of these polymorphisms in human populations , the use of W-CGH could be pertinent and of clinical relevance to assess rapidly , from a chromosomal viewpoint , genome similarities and differences in closely related genomes such as those of relatives , or in more specific situations such as bone marrow transplantation where chimerism is produced in the recipient .
	manualset3
218965	15	420337	7	NULL	NULL	0	NULL	chimerism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although further studies are necessary to corroborate and assess the overall incidence of these polymorphisms in human populations , the use of W-CGH could be pertinent and of clinical relevance to assess rapidly , from a chromosomal viewpoint , genome similarities and differences in closely related genomes such as those of relatives , or in more specific situations such as bone marrow transplantation where chimerism is produced in the recipient .
	manualset3
218966	16	420337	7	NULL	NULL	0	NULL	recipient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Although further studies are necessary to corroborate and assess the overall incidence of these polymorphisms in human populations , the use of W-CGH could be pertinent and of clinical relevance to assess rapidly , from a chromosomal viewpoint , genome similarities and differences in closely related genomes such as those of relatives , or in more specific situations such as bone marrow transplantation where chimerism is produced in the recipient .
	manualset3
218967	1	420338	7	NULL	NULL	0	NULL	FLT3 wild-type patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	FLT3 wild-type patients achieving an MRD ( - ) status , had a better outcome than those who remained MRD ( + ) ( 4-year RFS , 54 % vs 17 % P & lt ; .001 ; OS , 60 % vs 23 % , P = .002 ) .
	manualset3
218968	2	420338	7	NULL	NULL	0	NULL	MRD ( - ) status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	FLT3 wild-type patients achieving an MRD ( - ) status , had a better outcome than those who remained MRD ( + ) ( 4-year RFS , 54 % vs 17 % P & lt ; .001 ; OS , 60 % vs 23 % , P = .002 ) .
	manualset3
218969	3	420338	7	NULL	NULL	0	NULL	outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	FLT3 wild-type patients achieving an MRD ( - ) status , had a better outcome than those who remained MRD ( + ) ( 4-year RFS , 54 % vs 17 % P & lt ; .001 ; OS , 60 % vs 23 % , P = .002 ) .
	manualset3
218970	4	420338	7	NULL	NULL	0	NULL	MRD ( + )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	FLT3 wild-type patients achieving an MRD ( - ) status , had a better outcome than those who remained MRD ( + ) ( 4-year RFS , 54 % vs 17 % P & lt ; .001 ; OS , 60 % vs 23 % , P = .002 ) .
	manualset3
218971	5	420338	7	NULL	NULL	0	NULL	4-year RFS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	FLT3 wild-type patients achieving an MRD ( - ) status , had a better outcome than those who remained MRD ( + ) ( 4-year RFS , 54 % vs 17 % P & lt ; .001 ; OS , 60 % vs 23 % , P = .002 ) .
	manualset3
218972	6	420338	7	NULL	NULL	0	NULL	54 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	FLT3 wild-type patients achieving an MRD ( - ) status , had a better outcome than those who remained MRD ( + ) ( 4-year RFS , 54 % vs 17 % P & lt ; .001 ; OS , 60 % vs 23 % , P = .002 ) .
	manualset3
218973	7	420338	7	NULL	NULL	0	NULL	17 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	FLT3 wild-type patients achieving an MRD ( - ) status , had a better outcome than those who remained MRD ( + ) ( 4-year RFS , 54 % vs 17 % P & lt ; .001 ; OS , 60 % vs 23 % , P = .002 ) .
	manualset3
218974	8	420338	7	NULL	NULL	0	NULL	P & lt ; .001	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	FLT3 wild-type patients achieving an MRD ( - ) status , had a better outcome than those who remained MRD ( + ) ( 4-year RFS , 54 % vs 17 % P & lt ; .001 ; OS , 60 % vs 23 % , P = .002 ) .
	manualset3
218975	9	420338	7	NULL	NULL	0	NULL	OS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	FLT3 wild-type patients achieving an MRD ( - ) status , had a better outcome than those who remained MRD ( + ) ( 4-year RFS , 54 % vs 17 % P & lt ; .001 ; OS , 60 % vs 23 % , P = .002 ) .
	manualset3
218976	10	420338	7	NULL	NULL	0	NULL	 60 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	FLT3 wild-type patients achieving an MRD ( - ) status , had a better outcome than those who remained MRD ( + ) ( 4-year RFS , 54 % vs 17 % P & lt ; .001 ; OS , 60 % vs 23 % , P = .002 ) .
	manualset3
218977	11	420338	7	NULL	NULL	0	NULL	23 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	FLT3 wild-type patients achieving an MRD ( - ) status , had a better outcome than those who remained MRD ( + ) ( 4-year RFS , 54 % vs 17 % P & lt ; .001 ; OS , 60 % vs 23 % , P = .002 ) .
	manualset3
218978	12	420338	7	NULL	NULL	0	NULL	P = .002	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	FLT3 wild-type patients achieving an MRD ( - ) status , had a better outcome than those who remained MRD ( + ) ( 4-year RFS , 54 % vs 17 % P & lt ; .001 ; OS , 60 % vs 23 % , P = .002 ) .
	manualset3
218979	1	420339	7	NULL	NULL	0	NULL	pyridyl rings	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The pyridyl and aryl rings in the title compound , C ( 16 ) H ( 15 ) NO ( 3 ) H ( 2 ) O , which are located at the ends of the propenone unit , are nearly coplanar with this unit ( dihedral angles = 3.74 ( 14 ) and 5.06 ( 13 ) , respectively ) ; the rings are inclined at an angle of 6.2 ( 1 ) with respect to each other .
	manualset3
218980	2	420339	7	NULL	NULL	0	NULL	aryl rings	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The pyridyl and aryl rings in the title compound , C ( 16 ) H ( 15 ) NO ( 3 ) H ( 2 ) O , which are located at the ends of the propenone unit , are nearly coplanar with this unit ( dihedral angles = 3.74 ( 14 ) and 5.06 ( 13 ) , respectively ) ; the rings are inclined at an angle of 6.2 ( 1 ) with respect to each other .
	manualset3
218981	3	420339	7	NULL	NULL	0	NULL	title compound 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The pyridyl and aryl rings in the title compound , C ( 16 ) H ( 15 ) NO ( 3 ) H ( 2 ) O , which are located at the ends of the propenone unit , are nearly coplanar with this unit ( dihedral angles = 3.74 ( 14 ) and 5.06 ( 13 ) , respectively ) ; the rings are inclined at an angle of 6.2 ( 1 ) with respect to each other .
	manualset3
218982	4	420339	7	NULL	NULL	0	NULL	C ( 16 ) H ( 15 ) NO ( 3 ) H ( 2 ) O 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The pyridyl and aryl rings in the title compound , C ( 16 ) H ( 15 ) NO ( 3 ) H ( 2 ) O , which are located at the ends of the propenone unit , are nearly coplanar with this unit ( dihedral angles = 3.74 ( 14 ) and 5.06 ( 13 ) , respectively ) ; the rings are inclined at an angle of 6.2 ( 1 ) with respect to each other .
	manualset3
218983	5	420339	7	NULL	NULL	0	NULL	ends of the propenone unit	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The pyridyl and aryl rings in the title compound , C ( 16 ) H ( 15 ) NO ( 3 ) H ( 2 ) O , which are located at the ends of the propenone unit , are nearly coplanar with this unit ( dihedral angles = 3.74 ( 14 ) and 5.06 ( 13 ) , respectively ) ; the rings are inclined at an angle of 6.2 ( 1 ) with respect to each other .
	manualset3
218984	6	420339	7	NULL	NULL	0	NULL	unit	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The pyridyl and aryl rings in the title compound , C ( 16 ) H ( 15 ) NO ( 3 ) H ( 2 ) O , which are located at the ends of the propenone unit , are nearly coplanar with this unit ( dihedral angles = 3.74 ( 14 ) and 5.06 ( 13 ) , respectively ) ; the rings are inclined at an angle of 6.2 ( 1 ) with respect to each other .
	manualset3
218985	7	420339	7	NULL	NULL	0	NULL	dihedral angles	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The pyridyl and aryl rings in the title compound , C ( 16 ) H ( 15 ) NO ( 3 ) H ( 2 ) O , which are located at the ends of the propenone unit , are nearly coplanar with this unit ( dihedral angles = 3.74 ( 14 ) and 5.06 ( 13 ) , respectively ) ; the rings are inclined at an angle of 6.2 ( 1 ) with respect to each other .
	manualset3
218986	8	420339	7	NULL	NULL	0	NULL	3.74 ( 14 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The pyridyl and aryl rings in the title compound , C ( 16 ) H ( 15 ) NO ( 3 ) H ( 2 ) O , which are located at the ends of the propenone unit , are nearly coplanar with this unit ( dihedral angles = 3.74 ( 14 ) and 5.06 ( 13 ) , respectively ) ; the rings are inclined at an angle of 6.2 ( 1 ) with respect to each other .
	manualset3
218987	9	420339	7	NULL	NULL	0	NULL	5.06 ( 13 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The pyridyl and aryl rings in the title compound , C ( 16 ) H ( 15 ) NO ( 3 ) H ( 2 ) O , which are located at the ends of the propenone unit , are nearly coplanar with this unit ( dihedral angles = 3.74 ( 14 ) and 5.06 ( 13 ) , respectively ) ; the rings are inclined at an angle of 6.2 ( 1 ) with respect to each other .
	manualset3
218988	10	420339	7	NULL	NULL	0	NULL	rings	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The pyridyl and aryl rings in the title compound , C ( 16 ) H ( 15 ) NO ( 3 ) H ( 2 ) O , which are located at the ends of the propenone unit , are nearly coplanar with this unit ( dihedral angles = 3.74 ( 14 ) and 5.06 ( 13 ) , respectively ) ; the rings are inclined at an angle of 6.2 ( 1 ) with respect to each other .
	manualset3
218989	11	420339	7	NULL	NULL	0	NULL	angle	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The pyridyl and aryl rings in the title compound , C ( 16 ) H ( 15 ) NO ( 3 ) H ( 2 ) O , which are located at the ends of the propenone unit , are nearly coplanar with this unit ( dihedral angles = 3.74 ( 14 ) and 5.06 ( 13 ) , respectively ) ; the rings are inclined at an angle of 6.2 ( 1 ) with respect to each other .
	manualset3
218990	12	420339	7	NULL	NULL	0	NULL	6.2 ( 1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The pyridyl and aryl rings in the title compound , C ( 16 ) H ( 15 ) NO ( 3 ) H ( 2 ) O , which are located at the ends of the propenone unit , are nearly coplanar with this unit ( dihedral angles = 3.74 ( 14 ) and 5.06 ( 13 ) , respectively ) ; the rings are inclined at an angle of 6.2 ( 1 ) with respect to each other .
	manualset3
218991	1	420340	7	NULL	NULL	0	NULL	Decontamination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Decontamination of water in wells of Vinnitsa with the use of measured chemical-releasing cartridge holders ) .
	manualset3
218992	2	420340	7	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Decontamination of water in wells of Vinnitsa with the use of measured chemical-releasing cartridge holders ) .
	manualset3
218993	3	420340	7	NULL	NULL	0	NULL	wells of Vinnitsa	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( Decontamination of water in wells of Vinnitsa with the use of measured chemical-releasing cartridge holders ) .
	manualset3
218994	4	420340	7	NULL	NULL	0	NULL	use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Decontamination of water in wells of Vinnitsa with the use of measured chemical-releasing cartridge holders ) .
	manualset3
218995	5	420340	7	NULL	NULL	0	NULL	chemical-releasing cartridge holders	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	( Decontamination of water in wells of Vinnitsa with the use of measured chemical-releasing cartridge holders ) .
	manualset3
219041	1	420341	7	NULL	NULL	0	NULL	toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although toxicity was probably mainly due to dissolved contaminants , agreement between chemical and biological evidence of pollution was best for the sediment compartment , whereas porewater and surface water showed a higher degree of variability .
	manualset3
219042	2	420341	7	NULL	NULL	0	NULL	dissolved contaminants	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although toxicity was probably mainly due to dissolved contaminants , agreement between chemical and biological evidence of pollution was best for the sediment compartment , whereas porewater and surface water showed a higher degree of variability .
	manualset3
219043	3	420341	7	NULL	NULL	0	NULL	agreement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although toxicity was probably mainly due to dissolved contaminants , agreement between chemical and biological evidence of pollution was best for the sediment compartment , whereas porewater and surface water showed a higher degree of variability .
	manualset3
219044	4	420341	7	NULL	NULL	0	NULL	chemical evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although toxicity was probably mainly due to dissolved contaminants , agreement between chemical and biological evidence of pollution was best for the sediment compartment , whereas porewater and surface water showed a higher degree of variability .
	manualset3
219045	5	420341	7	NULL	NULL	0	NULL	biological evidence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although toxicity was probably mainly due to dissolved contaminants , agreement between chemical and biological evidence of pollution was best for the sediment compartment , whereas porewater and surface water showed a higher degree of variability .
	manualset3
219046	6	420341	7	NULL	NULL	0	NULL	pollution	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Although toxicity was probably mainly due to dissolved contaminants , agreement between chemical and biological evidence of pollution was best for the sediment compartment , whereas porewater and surface water showed a higher degree of variability .
	manualset3
219047	7	420341	7	NULL	NULL	0	NULL	sediment compartment	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although toxicity was probably mainly due to dissolved contaminants , agreement between chemical and biological evidence of pollution was best for the sediment compartment , whereas porewater and surface water showed a higher degree of variability .
	manualset3
219048	8	420341	7	NULL	NULL	0	NULL	porewater 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although toxicity was probably mainly due to dissolved contaminants , agreement between chemical and biological evidence of pollution was best for the sediment compartment , whereas porewater and surface water showed a higher degree of variability .
	manualset3
219049	9	420341	7	NULL	NULL	0	NULL	surface water 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although toxicity was probably mainly due to dissolved contaminants , agreement between chemical and biological evidence of pollution was best for the sediment compartment , whereas porewater and surface water showed a higher degree of variability .
	manualset3
219050	10	420341	7	NULL	NULL	0	NULL	higher degree	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although toxicity was probably mainly due to dissolved contaminants , agreement between chemical and biological evidence of pollution was best for the sediment compartment , whereas porewater and surface water showed a higher degree of variability .
	manualset3
219051	11	420341	7	NULL	NULL	0	NULL	variability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although toxicity was probably mainly due to dissolved contaminants , agreement between chemical and biological evidence of pollution was best for the sediment compartment , whereas porewater and surface water showed a higher degree of variability .
	manualset3
219052	1	420342	7	NULL	NULL	0	NULL	Drosophila substrate adhesion molecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Drosophila substrate adhesion molecule : sequence of laminin B1 chain reveals domains of homology with mouse .
	manualset3
219053	2	420342	7	NULL	NULL	0	NULL	sequence	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Drosophila substrate adhesion molecule : sequence of laminin B1 chain reveals domains of homology with mouse .
	manualset3
219054	3	420342	7	NULL	NULL	0	NULL	laminin B1 chain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Drosophila substrate adhesion molecule : sequence of laminin B1 chain reveals domains of homology with mouse .
	manualset3
219055	4	420342	7	NULL	NULL	0	NULL	domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Drosophila substrate adhesion molecule : sequence of laminin B1 chain reveals domains of homology with mouse .
	manualset3
219056	5	420342	7	NULL	NULL	0	NULL	homology	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Drosophila substrate adhesion molecule : sequence of laminin B1 chain reveals domains of homology with mouse .
	manualset3
219057	6	420342	7	NULL	NULL	0	NULL	mouse	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Drosophila substrate adhesion molecule : sequence of laminin B1 chain reveals domains of homology with mouse .
	manualset3
219058	1	420343	7	NULL	NULL	0	NULL	Fludarabine phosphate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Fludarabine phosphate was given as a 5 day bolus infusion to eleven evaluable patients with recurrent small cell lung carcinoma .
	manualset3
219059	2	420343	7	NULL	NULL	0	NULL	5 day	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Fludarabine phosphate was given as a 5 day bolus infusion to eleven evaluable patients with recurrent small cell lung carcinoma .
	manualset3
219060	3	420343	7	NULL	NULL	0	NULL	bolus infusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Fludarabine phosphate was given as a 5 day bolus infusion to eleven evaluable patients with recurrent small cell lung carcinoma .
	manualset3
219061	4	420343	7	NULL	NULL	0	NULL	eleven evaluable patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Fludarabine phosphate was given as a 5 day bolus infusion to eleven evaluable patients with recurrent small cell lung carcinoma .
	manualset3
219062	5	420343	7	NULL	NULL	0	NULL	recurrent small cell lung carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Fludarabine phosphate was given as a 5 day bolus infusion to eleven evaluable patients with recurrent small cell lung carcinoma .
	manualset3
219063	1	420344	7	NULL	NULL	0	NULL	Caffeine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Caffeine ( 1 mM ) , given either continuously or during the last 4 hours of the radiation exposure , counteracted the growth inhibition and G2 accumulation and enhanced cell killing .
	manualset3
219064	2	420344	7	NULL	NULL	0	NULL	1 mM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Caffeine ( 1 mM ) , given either continuously or during the last 4 hours of the radiation exposure , counteracted the growth inhibition and G2 accumulation and enhanced cell killing .
	manualset3
219065	3	420344	7	NULL	NULL	0	NULL	last 4 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Caffeine ( 1 mM ) , given either continuously or during the last 4 hours of the radiation exposure , counteracted the growth inhibition and G2 accumulation and enhanced cell killing .
	manualset3
219066	4	420344	7	NULL	NULL	0	NULL	radiation exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Caffeine ( 1 mM ) , given either continuously or during the last 4 hours of the radiation exposure , counteracted the growth inhibition and G2 accumulation and enhanced cell killing .
	manualset3
219067	5	420344	7	NULL	NULL	0	NULL	growth inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Caffeine ( 1 mM ) , given either continuously or during the last 4 hours of the radiation exposure , counteracted the growth inhibition and G2 accumulation and enhanced cell killing .
	manualset3
219068	6	420344	7	NULL	NULL	0	NULL	G2 accumulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Caffeine ( 1 mM ) , given either continuously or during the last 4 hours of the radiation exposure , counteracted the growth inhibition and G2 accumulation and enhanced cell killing .
	manualset3
219069	7	420344	7	NULL	NULL	0	NULL	cell killing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Caffeine ( 1 mM ) , given either continuously or during the last 4 hours of the radiation exposure , counteracted the growth inhibition and G2 accumulation and enhanced cell killing .
	manualset3
219075	1	420345	7	NULL	NULL	0	NULL	weight gain 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A weight gain could also be observed in this group but this gain was lower than those observed in the first two groups .
	manualset3
219077	2	420345	7	NULL	NULL	0	NULL	 group 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A weight gain could also be observed in this group but this gain was lower than those observed in the first two groups .
	manualset3
219079	3	420345	7	NULL	NULL	0	NULL	gain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A weight gain could also be observed in this group but this gain was lower than those observed in the first two groups .
	manualset3
219080	4	420345	7	NULL	NULL	0	NULL	first two groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A weight gain could also be observed in this group but this gain was lower than those observed in the first two groups .
	manualset3
219081	1	420346	7	NULL	NULL	0	NULL	 whole series 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the whole series the probability of seven-year survival was 0.65 ; 42 patients ( 31 % ) died from tumor disease .
	manualset3
219082	2	420346	7	NULL	NULL	0	NULL	probability	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the whole series the probability of seven-year survival was 0.65 ; 42 patients ( 31 % ) died from tumor disease .
	manualset3
219083	3	420346	7	NULL	NULL	0	NULL	seven-year survival 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For the whole series the probability of seven-year survival was 0.65 ; 42 patients ( 31 % ) died from tumor disease .
	manualset3
219084	4	420346	7	NULL	NULL	0	NULL	 0.65	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the whole series the probability of seven-year survival was 0.65 ; 42 patients ( 31 % ) died from tumor disease .
	manualset3
219086	5	420346	7	NULL	NULL	0	NULL	42 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	For the whole series the probability of seven-year survival was 0.65 ; 42 patients ( 31 % ) died from tumor disease .
	manualset3
219087	6	420346	7	NULL	NULL	0	NULL	31 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the whole series the probability of seven-year survival was 0.65 ; 42 patients ( 31 % ) died from tumor disease .
	manualset3
219088	7	420346	7	NULL	NULL	0	NULL	tumor disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	For the whole series the probability of seven-year survival was 0.65 ; 42 patients ( 31 % ) died from tumor disease .
	manualset3
219093	1	420347	7	NULL	NULL	0	NULL	 avoidance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , avoidance of hypoglycemia during intensive insulin therapy may be a key issue in effective tight glycemic control .
	manualset3
219094	2	420347	7	NULL	NULL	0	NULL	hypoglycemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , avoidance of hypoglycemia during intensive insulin therapy may be a key issue in effective tight glycemic control .
	manualset3
219097	3	420347	7	NULL	NULL	0	NULL	intensive insulin therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , avoidance of hypoglycemia during intensive insulin therapy may be a key issue in effective tight glycemic control .
	manualset3
219098	4	420347	7	NULL	NULL	NULL	NULL	key issue 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , avoidance of hypoglycemia during intensive insulin therapy may be a key issue in effective tight glycemic control .
	manualset3
219099	5	420347	7	NULL	NULL	0	NULL	effective tight glycemic control 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , avoidance of hypoglycemia during intensive insulin therapy may be a key issue in effective tight glycemic control .
	manualset3
219100	1	420348	7	NULL	NULL	0	NULL	transgenic rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although transgenic rats were normotensive and euglycemic and had a renal angiotensin II ( AngII ) level that was comparable to that of wild-type rats , transgenic rats developed proteinuria with aging and significant glomerulosclerosis at 28 wk of age .
	manualset3
219101	2	420348	7	NULL	NULL	0	NULL	euglycemic	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although transgenic rats were normotensive and euglycemic and had a renal angiotensin II ( AngII ) level that was comparable to that of wild-type rats , transgenic rats developed proteinuria with aging and significant glomerulosclerosis at 28 wk of age .
	manualset3
219102	3	420348	7	NULL	NULL	0	NULL	renal angiotensin II ( AngII ) level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although transgenic rats were normotensive and euglycemic and had a renal angiotensin II ( AngII ) level that was comparable to that of wild-type rats , transgenic rats developed proteinuria with aging and significant glomerulosclerosis at 28 wk of age .
	manualset3
219103	4	420348	7	NULL	NULL	0	NULL	wild-type rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although transgenic rats were normotensive and euglycemic and had a renal angiotensin II ( AngII ) level that was comparable to that of wild-type rats , transgenic rats developed proteinuria with aging and significant glomerulosclerosis at 28 wk of age .
	manualset3
219104	5	420348	7	NULL	NULL	0	NULL	transgenic rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although transgenic rats were normotensive and euglycemic and had a renal angiotensin II ( AngII ) level that was comparable to that of wild-type rats , transgenic rats developed proteinuria with aging and significant glomerulosclerosis at 28 wk of age .
	manualset3
219105	6	420348	7	NULL	NULL	NULL	NULL	proteinuria 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although transgenic rats were normotensive and euglycemic and had a renal angiotensin II ( AngII ) level that was comparable to that of wild-type rats , transgenic rats developed proteinuria with aging and significant glomerulosclerosis at 28 wk of age .
	manualset3
219106	7	420348	7	NULL	NULL	0	NULL	aging	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although transgenic rats were normotensive and euglycemic and had a renal angiotensin II ( AngII ) level that was comparable to that of wild-type rats , transgenic rats developed proteinuria with aging and significant glomerulosclerosis at 28 wk of age .
	manualset3
219107	8	420348	7	NULL	NULL	0	NULL	glomerulosclerosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Although transgenic rats were normotensive and euglycemic and had a renal angiotensin II ( AngII ) level that was comparable to that of wild-type rats , transgenic rats developed proteinuria with aging and significant glomerulosclerosis at 28 wk of age .
	manualset3
219108	9	420348	7	NULL	NULL	NULL	NULL	28 wk of age	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although transgenic rats were normotensive and euglycemic and had a renal angiotensin II ( AngII ) level that was comparable to that of wild-type rats , transgenic rats developed proteinuria with aging and significant glomerulosclerosis at 28 wk of age .
	manualset3
219111	1	420349	7	NULL	NULL	0	NULL	184 indoor patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	184 indoor patients suffering from various hepatic as well as non-hepatic disorders admitted in Kasturba Medical College & Hospital , Manipal during the year 1989 were studied for the presence of HBs Ag and anti HBs by ELISA .
	manualset3
219113	2	420349	7	NULL	NULL	0	NULL	hepatic disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	184 indoor patients suffering from various hepatic as well as non-hepatic disorders admitted in Kasturba Medical College & Hospital , Manipal during the year 1989 were studied for the presence of HBs Ag and anti HBs by ELISA .
	manualset3
219116	3	420349	7	NULL	NULL	0	NULL	non-hepatic disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	184 indoor patients suffering from various hepatic as well as non-hepatic disorders admitted in Kasturba Medical College & Hospital , Manipal during the year 1989 were studied for the presence of HBs Ag and anti HBs by ELISA .
	manualset3
219118	4	420349	7	NULL	NULL	0	NULL	Kasturba Medical College & Hospital	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	184 indoor patients suffering from various hepatic as well as non-hepatic disorders admitted in Kasturba Medical College & Hospital , Manipal during the year 1989 were studied for the presence of HBs Ag and anti HBs by ELISA .
	manualset3
219120	5	420349	7	NULL	NULL	0	NULL	Manipal	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	184 indoor patients suffering from various hepatic as well as non-hepatic disorders admitted in Kasturba Medical College & Hospital , Manipal during the year 1989 were studied for the presence of HBs Ag and anti HBs by ELISA .
	manualset3
219121	6	420349	7	NULL	NULL	NULL	NULL	year 1989	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	184 indoor patients suffering from various hepatic as well as non-hepatic disorders admitted in Kasturba Medical College & Hospital , Manipal during the year 1989 were studied for the presence of HBs Ag and anti HBs by ELISA .
	manualset3
219122	7	420349	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	184 indoor patients suffering from various hepatic as well as non-hepatic disorders admitted in Kasturba Medical College & Hospital , Manipal during the year 1989 were studied for the presence of HBs Ag and anti HBs by ELISA .
	manualset3
219123	8	420349	7	NULL	NULL	NULL	NULL	HBs Ag	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	184 indoor patients suffering from various hepatic as well as non-hepatic disorders admitted in Kasturba Medical College & Hospital , Manipal during the year 1989 were studied for the presence of HBs Ag and anti HBs by ELISA .
	manualset3
219124	9	420349	7	NULL	NULL	0	NULL	anti HBs	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	184 indoor patients suffering from various hepatic as well as non-hepatic disorders admitted in Kasturba Medical College & Hospital , Manipal during the year 1989 were studied for the presence of HBs Ag and anti HBs by ELISA .
	manualset3
219125	10	420349	7	NULL	NULL	0	NULL	ELISA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	184 indoor patients suffering from various hepatic as well as non-hepatic disorders admitted in Kasturba Medical College & Hospital , Manipal during the year 1989 were studied for the presence of HBs Ag and anti HBs by ELISA .
	manualset3
219126	1	420350	7	NULL	NULL	0	NULL	real crossed allergenicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If there is a real crossed allergenicity between pork meat and cat epithelia , we suggest that this crossed allergenicity is without doubt much greater and concerns more the meats and epithelia of mammals .
	manualset3
219127	2	420350	7	NULL	NULL	0	NULL	pork meat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	If there is a real crossed allergenicity between pork meat and cat epithelia , we suggest that this crossed allergenicity is without doubt much greater and concerns more the meats and epithelia of mammals .
	manualset3
219128	3	420350	7	NULL	NULL	0	NULL	cat epithelia	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	If there is a real crossed allergenicity between pork meat and cat epithelia , we suggest that this crossed allergenicity is without doubt much greater and concerns more the meats and epithelia of mammals .
	manualset3
219129	4	420350	7	NULL	NULL	0	NULL	crossed allergenicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	If there is a real crossed allergenicity between pork meat and cat epithelia , we suggest that this crossed allergenicity is without doubt much greater and concerns more the meats and epithelia of mammals .
	manualset3
219130	5	420350	7	NULL	NULL	0	NULL	meats 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	If there is a real crossed allergenicity between pork meat and cat epithelia , we suggest that this crossed allergenicity is without doubt much greater and concerns more the meats and epithelia of mammals .
	manualset3
219131	6	420350	7	NULL	NULL	0	NULL	epithelia of mammals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	If there is a real crossed allergenicity between pork meat and cat epithelia , we suggest that this crossed allergenicity is without doubt much greater and concerns more the meats and epithelia of mammals .
	manualset3
219138	1	420351	7	NULL	NULL	0	NULL	 long HCl treatment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After long HCl treatment , DNA is barely detectable by osmium ammine while phosphorus is still present in the thin sections .
	manualset3
219139	2	420351	7	NULL	NULL	0	NULL	DNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	After long HCl treatment , DNA is barely detectable by osmium ammine while phosphorus is still present in the thin sections .
	manualset3
219140	3	420351	7	NULL	NULL	0	NULL	osmium ammine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After long HCl treatment , DNA is barely detectable by osmium ammine while phosphorus is still present in the thin sections .
	manualset3
219141	4	420351	7	NULL	NULL	0	NULL	phosphorus	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After long HCl treatment , DNA is barely detectable by osmium ammine while phosphorus is still present in the thin sections .
	manualset3
219142	5	420351	7	NULL	NULL	0	NULL	thin sections 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	After long HCl treatment , DNA is barely detectable by osmium ammine while phosphorus is still present in the thin sections .
	manualset3
219143	1	420352	7	NULL	NULL	0	NULL	imidazolium cations	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The imidazolium cations link these sheets peripherally down c through carboxyl-ate O-H-N and N ' - HO ( hy-droxy ) bridges , giving a three-dimensional framework structure .
	manualset3
219144	2	420352	7	NULL	NULL	0	NULL	 sheets	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The imidazolium cations link these sheets peripherally down c through carboxyl-ate O-H-N and N ' - HO ( hy-droxy ) bridges , giving a three-dimensional framework structure .
	manualset3
219146	3	420352	7	NULL	NULL	0	NULL	carboxyl-ate O-H-N bridge	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The imidazolium cations link these sheets peripherally down c through carboxyl-ate O-H-N and N ' - HO ( hy-droxy ) bridges , giving a three-dimensional framework structure .
	manualset3
219149	4	420352	7	NULL	NULL	NULL	NULL	N ' - HO ( hy-droxy ) bridges	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The imidazolium cations link these sheets peripherally down c through carboxyl-ate O-H-N and N ' - HO ( hy-droxy ) bridges , giving a three-dimensional framework structure .
	manualset3
219150	5	420352	7	NULL	NULL	0	NULL	three-dimensional framework structure 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The imidazolium cations link these sheets peripherally down c through carboxyl-ate O-H-N and N ' - HO ( hy-droxy ) bridges , giving a three-dimensional framework structure .
	manualset3
219151	1	420353	7	NULL	NULL	0	NULL	 two olfactory systems	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Even though these two olfactory systems are functionally and anatomically separate , their sensory neurons show a common mechanism of receptor gene regulation : each neuron expresses a single receptor gene from a single allele .
	manualset3
219152	2	420353	7	NULL	NULL	0	NULL	sensory neurons	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Even though these two olfactory systems are functionally and anatomically separate , their sensory neurons show a common mechanism of receptor gene regulation : each neuron expresses a single receptor gene from a single allele .
	manualset3
219153	3	420353	7	NULL	NULL	0	NULL	common mechanism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Even though these two olfactory systems are functionally and anatomically separate , their sensory neurons show a common mechanism of receptor gene regulation : each neuron expresses a single receptor gene from a single allele .
	manualset3
219155	4	420353	7	NULL	NULL	0	NULL	receptor gene regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Even though these two olfactory systems are functionally and anatomically separate , their sensory neurons show a common mechanism of receptor gene regulation : each neuron expresses a single receptor gene from a single allele .
	manualset3
219156	5	420353	7	NULL	NULL	0	NULL	neuron	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Even though these two olfactory systems are functionally and anatomically separate , their sensory neurons show a common mechanism of receptor gene regulation : each neuron expresses a single receptor gene from a single allele .
	manualset3
219157	6	420353	7	NULL	NULL	0	NULL	single receptor gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Even though these two olfactory systems are functionally and anatomically separate , their sensory neurons show a common mechanism of receptor gene regulation : each neuron expresses a single receptor gene from a single allele .
	manualset3
219158	7	420353	7	NULL	NULL	0	NULL	single allele	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Even though these two olfactory systems are functionally and anatomically separate , their sensory neurons show a common mechanism of receptor gene regulation : each neuron expresses a single receptor gene from a single allele .
	manualset3
219171	1	420354	7	NULL	NULL	0	NULL	second high potential heme 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The second high potential heme , H2 ( +240 mV ) , peaks at 554 nm and makes a tilt of 55 degrees with the membrane .
	manualset3
219172	2	420354	7	NULL	NULL	0	NULL	H2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The second high potential heme , H2 ( +240 mV ) , peaks at 554 nm and makes a tilt of 55 degrees with the membrane .
	manualset3
219173	3	420354	7	NULL	NULL	0	NULL	+240 mV	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The second high potential heme , H2 ( +240 mV ) , peaks at 554 nm and makes a tilt of 55 degrees with the membrane .
	manualset3
219174	4	420354	7	NULL	NULL	0	NULL	 554 nm 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The second high potential heme , H2 ( +240 mV ) , peaks at 554 nm and makes a tilt of 55 degrees with the membrane .
	manualset3
219175	5	420354	7	NULL	NULL	0	NULL	tilt 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The second high potential heme , H2 ( +240 mV ) , peaks at 554 nm and makes a tilt of 55 degrees with the membrane .
	manualset3
219176	6	420354	7	NULL	NULL	0	NULL	55 degrees	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The second high potential heme , H2 ( +240 mV ) , peaks at 554 nm and makes a tilt of 55 degrees with the membrane .
	manualset3
219177	7	420354	7	NULL	NULL	0	NULL	membrane 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The second high potential heme , H2 ( +240 mV ) , peaks at 554 nm and makes a tilt of 55 degrees with the membrane .
	manualset3
219178	1	420355	7	NULL	NULL	0	NULL	 present data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data suggest an epistatic action of ACP1 concerning the effect of Hp on the susceptibility to convulsive disorders .
	manualset3
219179	2	420355	7	NULL	NULL	0	NULL	epistatic action 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data suggest an epistatic action of ACP1 concerning the effect of Hp on the susceptibility to convulsive disorders .
	manualset3
219180	3	420355	7	NULL	NULL	0	NULL	ACP1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data suggest an epistatic action of ACP1 concerning the effect of Hp on the susceptibility to convulsive disorders .
	manualset3
219181	4	420355	7	NULL	NULL	0	NULL	effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data suggest an epistatic action of ACP1 concerning the effect of Hp on the susceptibility to convulsive disorders .
	manualset3
219182	5	420355	7	NULL	NULL	0	NULL	Hp	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data suggest an epistatic action of ACP1 concerning the effect of Hp on the susceptibility to convulsive disorders .
	manualset3
219183	6	420355	7	NULL	NULL	0	NULL	susceptibility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data suggest an epistatic action of ACP1 concerning the effect of Hp on the susceptibility to convulsive disorders .
	manualset3
219184	7	420355	7	NULL	NULL	0	NULL	convulsive disorders 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data suggest an epistatic action of ACP1 concerning the effect of Hp on the susceptibility to convulsive disorders .
	manualset3
219185	1	420356	7	NULL	NULL	NULL	NULL	inferior vena cava ( IVC ) filters	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although use of inferior vena cava ( IVC ) filters for prophylaxis against pulmonary embolism ( PE ) is well reported in adults , long-term studies in children are lacking .
	manualset3
219186	2	420356	7	NULL	NULL	NULL	NULL	prophylaxis 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although use of inferior vena cava ( IVC ) filters for prophylaxis against pulmonary embolism ( PE ) is well reported in adults , long-term studies in children are lacking .
	manualset3
219187	3	420356	7	NULL	NULL	0	NULL	pulmonary embolism ( PE )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Although use of inferior vena cava ( IVC ) filters for prophylaxis against pulmonary embolism ( PE ) is well reported in adults , long-term studies in children are lacking .
	manualset3
219188	4	420356	7	NULL	NULL	0	NULL	adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although use of inferior vena cava ( IVC ) filters for prophylaxis against pulmonary embolism ( PE ) is well reported in adults , long-term studies in children are lacking .
	manualset3
219189	5	420356	7	NULL	NULL	0	NULL	long-term studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although use of inferior vena cava ( IVC ) filters for prophylaxis against pulmonary embolism ( PE ) is well reported in adults , long-term studies in children are lacking .
	manualset3
219190	6	420356	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although use of inferior vena cava ( IVC ) filters for prophylaxis against pulmonary embolism ( PE ) is well reported in adults , long-term studies in children are lacking .
	manualset3
221085	7	420356	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although use of inferior vena cava ( IVC ) filters for prophylaxis against pulmonary embolism ( PE ) is well reported in adults , long-term studies in children are lacking .
	manualset3
219191	1	420357	7	NULL	NULL	0	NULL	SNX rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In these SNX rats , left , but not right , ventricular beta-adrenoceptor density was significantly reduced , and membrane-associated G-protein-coupled receptor kinase activity was significantly increased compared with sham-operated rats .
	manualset3
219192	2	420357	7	NULL	NULL	NULL	NULL	left ventricular beta-adrenoceptor density	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In these SNX rats , left , but not right , ventricular beta-adrenoceptor density was significantly reduced , and membrane-associated G-protein-coupled receptor kinase activity was significantly increased compared with sham-operated rats .
	manualset3
219193	3	420357	7	NULL	NULL	0	NULL	membrane-associated G-protein-coupled receptor kinase activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In these SNX rats , left , but not right , ventricular beta-adrenoceptor density was significantly reduced , and membrane-associated G-protein-coupled receptor kinase activity was significantly increased compared with sham-operated rats .
	manualset3
219194	4	420357	7	NULL	NULL	0	NULL	sham-operated rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In these SNX rats , left , but not right , ventricular beta-adrenoceptor density was significantly reduced , and membrane-associated G-protein-coupled receptor kinase activity was significantly increased compared with sham-operated rats .
	manualset3
219195	1	420358	7	NULL	NULL	0	NULL	capability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We investigated the capability of recombinant cathepsin S propeptide to catalyze the renaturation of denatured mature cathepsin S. The experiments showed a 10-25 fold faster renaturation rate in presence than in absence of the propeptide underlining its function as intramolecular chaperone .
	manualset3
219196	2	420358	7	NULL	NULL	0	NULL	recombinant cathepsin S propeptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	We investigated the capability of recombinant cathepsin S propeptide to catalyze the renaturation of denatured mature cathepsin S. The experiments showed a 10-25 fold faster renaturation rate in presence than in absence of the propeptide underlining its function as intramolecular chaperone .
	manualset3
219197	3	420358	7	NULL	NULL	0	NULL	renaturation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We investigated the capability of recombinant cathepsin S propeptide to catalyze the renaturation of denatured mature cathepsin S. The experiments showed a 10-25 fold faster renaturation rate in presence than in absence of the propeptide underlining its function as intramolecular chaperone .
	manualset3
219198	4	420358	7	NULL	NULL	0	NULL	denatured mature cathepsin S	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We investigated the capability of recombinant cathepsin S propeptide to catalyze the renaturation of denatured mature cathepsin S. The experiments showed a 10-25 fold faster renaturation rate in presence than in absence of the propeptide underlining its function as intramolecular chaperone .
	manualset3
219199	5	420358	7	NULL	NULL	0	NULL	experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We investigated the capability of recombinant cathepsin S propeptide to catalyze the renaturation of denatured mature cathepsin S. The experiments showed a 10-25 fold faster renaturation rate in presence than in absence of the propeptide underlining its function as intramolecular chaperone .
	manualset3
219200	6	420358	7	NULL	NULL	0	NULL	10-25 fold 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We investigated the capability of recombinant cathepsin S propeptide to catalyze the renaturation of denatured mature cathepsin S. The experiments showed a 10-25 fold faster renaturation rate in presence than in absence of the propeptide underlining its function as intramolecular chaperone .
	manualset3
219201	7	420358	7	NULL	NULL	0	NULL	faster renaturation rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We investigated the capability of recombinant cathepsin S propeptide to catalyze the renaturation of denatured mature cathepsin S. The experiments showed a 10-25 fold faster renaturation rate in presence than in absence of the propeptide underlining its function as intramolecular chaperone .
	manualset3
219202	8	420358	7	NULL	NULL	0	NULL	 presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We investigated the capability of recombinant cathepsin S propeptide to catalyze the renaturation of denatured mature cathepsin S. The experiments showed a 10-25 fold faster renaturation rate in presence than in absence of the propeptide underlining its function as intramolecular chaperone .
	manualset3
219203	9	420358	7	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We investigated the capability of recombinant cathepsin S propeptide to catalyze the renaturation of denatured mature cathepsin S. The experiments showed a 10-25 fold faster renaturation rate in presence than in absence of the propeptide underlining its function as intramolecular chaperone .
	manualset3
219204	10	420358	7	NULL	NULL	0	NULL	propeptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	We investigated the capability of recombinant cathepsin S propeptide to catalyze the renaturation of denatured mature cathepsin S. The experiments showed a 10-25 fold faster renaturation rate in presence than in absence of the propeptide underlining its function as intramolecular chaperone .
	manualset3
219205	11	420358	7	NULL	NULL	0	NULL	 function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We investigated the capability of recombinant cathepsin S propeptide to catalyze the renaturation of denatured mature cathepsin S. The experiments showed a 10-25 fold faster renaturation rate in presence than in absence of the propeptide underlining its function as intramolecular chaperone .
	manualset3
219206	12	420358	7	NULL	NULL	0	NULL	intramolecular chaperone	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	We investigated the capability of recombinant cathepsin S propeptide to catalyze the renaturation of denatured mature cathepsin S. The experiments showed a 10-25 fold faster renaturation rate in presence than in absence of the propeptide underlining its function as intramolecular chaperone .
	manualset3
219207	1	420359	7	NULL	NULL	0	NULL	 standard IVM	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Following standard IVM and IVF , zygotes were cultured in modified synthetic oviduct fluid ( SOF ) , with 10 % fetal calf serum ( FCS ) added 48 hr post insemination , in a humidified atmosphere of 5 % CO2 , 5 % O2 and 90 % N2 .
	manualset3
219208	2	420359	7	NULL	NULL	0	NULL	 standard IVF	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Following standard IVM and IVF , zygotes were cultured in modified synthetic oviduct fluid ( SOF ) , with 10 % fetal calf serum ( FCS ) added 48 hr post insemination , in a humidified atmosphere of 5 % CO2 , 5 % O2 and 90 % N2 .
	manualset3
219209	3	420359	7	NULL	NULL	0	NULL	zygotes 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Following standard IVM and IVF , zygotes were cultured in modified synthetic oviduct fluid ( SOF ) , with 10 % fetal calf serum ( FCS ) added 48 hr post insemination , in a humidified atmosphere of 5 % CO2 , 5 % O2 and 90 % N2 .
	manualset3
219210	4	420359	7	NULL	NULL	0	NULL	modified synthetic oviduct fluid ( SOF )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Following standard IVM and IVF , zygotes were cultured in modified synthetic oviduct fluid ( SOF ) , with 10 % fetal calf serum ( FCS ) added 48 hr post insemination , in a humidified atmosphere of 5 % CO2 , 5 % O2 and 90 % N2 .
	manualset3
219211	5	420359	7	NULL	NULL	0	NULL	10 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Following standard IVM and IVF , zygotes were cultured in modified synthetic oviduct fluid ( SOF ) , with 10 % fetal calf serum ( FCS ) added 48 hr post insemination , in a humidified atmosphere of 5 % CO2 , 5 % O2 and 90 % N2 .
	manualset3
219212	6	420359	7	NULL	NULL	0	NULL	fetal calf serum ( FCS )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Following standard IVM and IVF , zygotes were cultured in modified synthetic oviduct fluid ( SOF ) , with 10 % fetal calf serum ( FCS ) added 48 hr post insemination , in a humidified atmosphere of 5 % CO2 , 5 % O2 and 90 % N2 .
	manualset3
219213	7	420359	7	NULL	NULL	0	NULL	 48 hr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Following standard IVM and IVF , zygotes were cultured in modified synthetic oviduct fluid ( SOF ) , with 10 % fetal calf serum ( FCS ) added 48 hr post insemination , in a humidified atmosphere of 5 % CO2 , 5 % O2 and 90 % N2 .
	manualset3
219214	8	420359	7	NULL	NULL	0	NULL	post insemination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Following standard IVM and IVF , zygotes were cultured in modified synthetic oviduct fluid ( SOF ) , with 10 % fetal calf serum ( FCS ) added 48 hr post insemination , in a humidified atmosphere of 5 % CO2 , 5 % O2 and 90 % N2 .
	manualset3
219215	9	420359	7	NULL	NULL	0	NULL	humidified atmosphere	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Following standard IVM and IVF , zygotes were cultured in modified synthetic oviduct fluid ( SOF ) , with 10 % fetal calf serum ( FCS ) added 48 hr post insemination , in a humidified atmosphere of 5 % CO2 , 5 % O2 and 90 % N2 .
	manualset3
219216	10	420359	7	NULL	NULL	0	NULL	5 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Following standard IVM and IVF , zygotes were cultured in modified synthetic oviduct fluid ( SOF ) , with 10 % fetal calf serum ( FCS ) added 48 hr post insemination , in a humidified atmosphere of 5 % CO2 , 5 % O2 and 90 % N2 .
	manualset3
219217	11	420359	7	NULL	NULL	0	NULL	CO2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Following standard IVM and IVF , zygotes were cultured in modified synthetic oviduct fluid ( SOF ) , with 10 % fetal calf serum ( FCS ) added 48 hr post insemination , in a humidified atmosphere of 5 % CO2 , 5 % O2 and 90 % N2 .
	manualset3
219218	12	420359	7	NULL	NULL	0	NULL	 5 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Following standard IVM and IVF , zygotes were cultured in modified synthetic oviduct fluid ( SOF ) , with 10 % fetal calf serum ( FCS ) added 48 hr post insemination , in a humidified atmosphere of 5 % CO2 , 5 % O2 and 90 % N2 .
	manualset3
219219	13	420359	7	NULL	NULL	0	NULL	O2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Following standard IVM and IVF , zygotes were cultured in modified synthetic oviduct fluid ( SOF ) , with 10 % fetal calf serum ( FCS ) added 48 hr post insemination , in a humidified atmosphere of 5 % CO2 , 5 % O2 and 90 % N2 .
	manualset3
219220	14	420359	7	NULL	NULL	0	NULL	90 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Following standard IVM and IVF , zygotes were cultured in modified synthetic oviduct fluid ( SOF ) , with 10 % fetal calf serum ( FCS ) added 48 hr post insemination , in a humidified atmosphere of 5 % CO2 , 5 % O2 and 90 % N2 .
	manualset3
219221	15	420359	7	NULL	NULL	0	NULL	N2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Following standard IVM and IVF , zygotes were cultured in modified synthetic oviduct fluid ( SOF ) , with 10 % fetal calf serum ( FCS ) added 48 hr post insemination , in a humidified atmosphere of 5 % CO2 , 5 % O2 and 90 % N2 .
	manualset3
219222	1	420360	7	NULL	NULL	NULL	NULL	Multiple molecular forms 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Multiple molecular forms of glia maturation factor .
	manualset3
219223	2	420360	7	NULL	NULL	0	NULL	glia maturation factor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple molecular forms of glia maturation factor .
	manualset3
219224	1	420361	7	NULL	NULL	0	NULL	MMP-9	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	MMP-9 was closely related with the invasion and metastasis of SACC .
	manualset3
219225	2	420361	7	NULL	NULL	0	NULL	 invasion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MMP-9 was closely related with the invasion and metastasis of SACC .
	manualset3
219226	3	420361	7	NULL	NULL	0	NULL	metastasis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MMP-9 was closely related with the invasion and metastasis of SACC .
	manualset3
219227	4	420361	7	NULL	NULL	0	NULL	SACC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	MMP-9 was closely related with the invasion and metastasis of SACC .
	manualset3
219228	1	420362	7	NULL	NULL	0	NULL	Measurement	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of fiber-cladding diameter uniformity by use of whispering-gallery modes : nanometer resolution in diameter variations along millimeter to centimeter lengths .
	manualset3
219229	2	420362	7	NULL	NULL	0	NULL	fiber-cladding diameter uniformity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of fiber-cladding diameter uniformity by use of whispering-gallery modes : nanometer resolution in diameter variations along millimeter to centimeter lengths .
	manualset3
219230	3	420362	7	NULL	NULL	0	NULL	whispering-gallery modes	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of fiber-cladding diameter uniformity by use of whispering-gallery modes : nanometer resolution in diameter variations along millimeter to centimeter lengths .
	manualset3
219231	4	420362	7	NULL	NULL	NULL	NULL	nanometer resolution	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Measurement of fiber-cladding diameter uniformity by use of whispering-gallery modes : nanometer resolution in diameter variations along millimeter to centimeter lengths .
	manualset3
219232	5	420362	7	NULL	NULL	NULL	NULL	diameter variations	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Measurement of fiber-cladding diameter uniformity by use of whispering-gallery modes : nanometer resolution in diameter variations along millimeter to centimeter lengths .
	manualset3
219233	6	420362	7	NULL	NULL	0	NULL	millimeter	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of fiber-cladding diameter uniformity by use of whispering-gallery modes : nanometer resolution in diameter variations along millimeter to centimeter lengths .
	manualset3
219234	7	420362	7	NULL	NULL	0	NULL	centimeter lengths	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of fiber-cladding diameter uniformity by use of whispering-gallery modes : nanometer resolution in diameter variations along millimeter to centimeter lengths .
	manualset3
219235	1	420363	7	NULL	NULL	0	NULL	 vascular calcification 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although vascular calcification is present in the vast majority of those aged over 70 years and causes serious cardiovascular dysfunction , strategies for its prevention and effective management are currently not available because the mechanism of its pathogenesis is unknown .
	manualset3
219236	2	420363	7	NULL	NULL	0	NULL	70 years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Although vascular calcification is present in the vast majority of those aged over 70 years and causes serious cardiovascular dysfunction , strategies for its prevention and effective management are currently not available because the mechanism of its pathogenesis is unknown .
	manualset3
219237	3	420363	7	NULL	NULL	0	NULL	serious cardiovascular dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although vascular calcification is present in the vast majority of those aged over 70 years and causes serious cardiovascular dysfunction , strategies for its prevention and effective management are currently not available because the mechanism of its pathogenesis is unknown .
	manualset3
219238	4	420363	7	NULL	NULL	0	NULL	strategies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although vascular calcification is present in the vast majority of those aged over 70 years and causes serious cardiovascular dysfunction , strategies for its prevention and effective management are currently not available because the mechanism of its pathogenesis is unknown .
	manualset3
219239	5	420363	7	NULL	NULL	NULL	NULL	prevention	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although vascular calcification is present in the vast majority of those aged over 70 years and causes serious cardiovascular dysfunction , strategies for its prevention and effective management are currently not available because the mechanism of its pathogenesis is unknown .
	manualset3
219240	6	420363	7	NULL	NULL	NULL	NULL	effective management	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although vascular calcification is present in the vast majority of those aged over 70 years and causes serious cardiovascular dysfunction , strategies for its prevention and effective management are currently not available because the mechanism of its pathogenesis is unknown .
	manualset3
219241	7	420363	7	NULL	NULL	NULL	NULL	mechanism 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although vascular calcification is present in the vast majority of those aged over 70 years and causes serious cardiovascular dysfunction , strategies for its prevention and effective management are currently not available because the mechanism of its pathogenesis is unknown .
	manualset3
219242	8	420363	7	NULL	NULL	0	NULL	pathogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although vascular calcification is present in the vast majority of those aged over 70 years and causes serious cardiovascular dysfunction , strategies for its prevention and effective management are currently not available because the mechanism of its pathogenesis is unknown .
	manualset3
220506	9	420363	7	NULL	NULL	0	NULL	vast majority	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although vascular calcification is present in the vast majority of those aged over 70 years and causes serious cardiovascular dysfunction , strategies for its prevention and effective management are currently not available because the mechanism of its pathogenesis is unknown .
	manualset3
219243	1	420364	7	NULL	NULL	0	NULL	generation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular we demonstrate the generation of square output pulses , which have the potential to significantly increase the maximum pulse energy extractable from an amplifier before the peak power reaches the threshold for SRS , and for high efficiency frequency conversion .
	manualset3
219244	2	420364	7	NULL	NULL	0	NULL	square output pulses	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular we demonstrate the generation of square output pulses , which have the potential to significantly increase the maximum pulse energy extractable from an amplifier before the peak power reaches the threshold for SRS , and for high efficiency frequency conversion .
	manualset3
219245	3	420364	7	NULL	NULL	0	NULL	maximum pulse energy 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular we demonstrate the generation of square output pulses , which have the potential to significantly increase the maximum pulse energy extractable from an amplifier before the peak power reaches the threshold for SRS , and for high efficiency frequency conversion .
	manualset3
219246	4	420364	7	NULL	NULL	0	NULL	amplifier	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular we demonstrate the generation of square output pulses , which have the potential to significantly increase the maximum pulse energy extractable from an amplifier before the peak power reaches the threshold for SRS , and for high efficiency frequency conversion .
	manualset3
219247	5	420364	7	NULL	NULL	0	NULL	peak power	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular we demonstrate the generation of square output pulses , which have the potential to significantly increase the maximum pulse energy extractable from an amplifier before the peak power reaches the threshold for SRS , and for high efficiency frequency conversion .
	manualset3
219248	6	420364	7	NULL	NULL	0	NULL	threshold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular we demonstrate the generation of square output pulses , which have the potential to significantly increase the maximum pulse energy extractable from an amplifier before the peak power reaches the threshold for SRS , and for high efficiency frequency conversion .
	manualset3
219249	7	420364	7	NULL	NULL	0	NULL	SRS	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular we demonstrate the generation of square output pulses , which have the potential to significantly increase the maximum pulse energy extractable from an amplifier before the peak power reaches the threshold for SRS , and for high efficiency frequency conversion .
	manualset3
219250	8	420364	7	NULL	NULL	0	NULL	high efficiency 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular we demonstrate the generation of square output pulses , which have the potential to significantly increase the maximum pulse energy extractable from an amplifier before the peak power reaches the threshold for SRS , and for high efficiency frequency conversion .
	manualset3
219251	9	420364	7	NULL	NULL	0	NULL	frequency conversion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular we demonstrate the generation of square output pulses , which have the potential to significantly increase the maximum pulse energy extractable from an amplifier before the peak power reaches the threshold for SRS , and for high efficiency frequency conversion .
	manualset3
219252	10	420364	7	NULL	NULL	0	NULL	potential	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular we demonstrate the generation of square output pulses , which have the potential to significantly increase the maximum pulse energy extractable from an amplifier before the peak power reaches the threshold for SRS , and for high efficiency frequency conversion .
	manualset3
219253	1	420365	7	NULL	NULL	0	NULL	Acute symptomatic pulmonary embolism	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute symptomatic pulmonary embolism associated with long haul air travel to Sydney .
	manualset3
219254	2	420365	7	NULL	NULL	0	NULL	 long haul air travel 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute symptomatic pulmonary embolism associated with long haul air travel to Sydney .
	manualset3
219255	3	420365	7	NULL	NULL	0	NULL	Sydney	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute symptomatic pulmonary embolism associated with long haul air travel to Sydney .
	manualset3
219256	1	420366	7	NULL	NULL	0	NULL	western dilemma 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The western dilemma : miners , silicosis , and compensation .
	manualset3
219257	2	420366	7	NULL	NULL	0	NULL	miners 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The western dilemma : miners , silicosis , and compensation .
	manualset3
219258	3	420366	7	NULL	NULL	0	NULL	silicosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The western dilemma : miners , silicosis , and compensation .
	manualset3
219259	4	420366	7	NULL	NULL	0	NULL	compensation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The western dilemma : miners , silicosis , and compensation .
	manualset3
219260	1	420367	7	NULL	NULL	0	NULL	similar levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , at similar levels of hypocapnia ( PaCO2 18-20 mmHg ) , CBF was significantly lower ( P less than 0.01 ) during administration of isoflurane-N2O ( 29.0 + / - 4.5 ml X 100 g-1 X min-1 ) than during administration of either N2O ( 40.6 + / - 5.5 ml X 100 g-1 X min-1 ) or halothane-N2O ( 39.6 + / - 7.8 ml X 100 g-1 X min-1 ) .
	manualset3
219261	2	420367	7	NULL	NULL	0	NULL	 hypocapnia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , at similar levels of hypocapnia ( PaCO2 18-20 mmHg ) , CBF was significantly lower ( P less than 0.01 ) during administration of isoflurane-N2O ( 29.0 + / - 4.5 ml X 100 g-1 X min-1 ) than during administration of either N2O ( 40.6 + / - 5.5 ml X 100 g-1 X min-1 ) or halothane-N2O ( 39.6 + / - 7.8 ml X 100 g-1 X min-1 ) .
	manualset3
219262	3	420367	7	NULL	NULL	0	NULL	PaCO2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , at similar levels of hypocapnia ( PaCO2 18-20 mmHg ) , CBF was significantly lower ( P less than 0.01 ) during administration of isoflurane-N2O ( 29.0 + / - 4.5 ml X 100 g-1 X min-1 ) than during administration of either N2O ( 40.6 + / - 5.5 ml X 100 g-1 X min-1 ) or halothane-N2O ( 39.6 + / - 7.8 ml X 100 g-1 X min-1 ) .
	manualset3
219263	4	420367	7	NULL	NULL	0	NULL	18-20 mmHg	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , at similar levels of hypocapnia ( PaCO2 18-20 mmHg ) , CBF was significantly lower ( P less than 0.01 ) during administration of isoflurane-N2O ( 29.0 + / - 4.5 ml X 100 g-1 X min-1 ) than during administration of either N2O ( 40.6 + / - 5.5 ml X 100 g-1 X min-1 ) or halothane-N2O ( 39.6 + / - 7.8 ml X 100 g-1 X min-1 ) .
	manualset3
219264	5	420367	7	NULL	NULL	0	NULL	CBF	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , at similar levels of hypocapnia ( PaCO2 18-20 mmHg ) , CBF was significantly lower ( P less than 0.01 ) during administration of isoflurane-N2O ( 29.0 + / - 4.5 ml X 100 g-1 X min-1 ) than during administration of either N2O ( 40.6 + / - 5.5 ml X 100 g-1 X min-1 ) or halothane-N2O ( 39.6 + / - 7.8 ml X 100 g-1 X min-1 ) .
	manualset3
219265	6	420367	7	NULL	NULL	0	NULL	P less than 0.01	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , at similar levels of hypocapnia ( PaCO2 18-20 mmHg ) , CBF was significantly lower ( P less than 0.01 ) during administration of isoflurane-N2O ( 29.0 + / - 4.5 ml X 100 g-1 X min-1 ) than during administration of either N2O ( 40.6 + / - 5.5 ml X 100 g-1 X min-1 ) or halothane-N2O ( 39.6 + / - 7.8 ml X 100 g-1 X min-1 ) .
	manualset3
219266	7	420367	7	NULL	NULL	0	NULL	administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , at similar levels of hypocapnia ( PaCO2 18-20 mmHg ) , CBF was significantly lower ( P less than 0.01 ) during administration of isoflurane-N2O ( 29.0 + / - 4.5 ml X 100 g-1 X min-1 ) than during administration of either N2O ( 40.6 + / - 5.5 ml X 100 g-1 X min-1 ) or halothane-N2O ( 39.6 + / - 7.8 ml X 100 g-1 X min-1 ) .
	manualset3
219267	8	420367	7	NULL	NULL	0	NULL	isoflurane-N2O	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , at similar levels of hypocapnia ( PaCO2 18-20 mmHg ) , CBF was significantly lower ( P less than 0.01 ) during administration of isoflurane-N2O ( 29.0 + / - 4.5 ml X 100 g-1 X min-1 ) than during administration of either N2O ( 40.6 + / - 5.5 ml X 100 g-1 X min-1 ) or halothane-N2O ( 39.6 + / - 7.8 ml X 100 g-1 X min-1 ) .
	manualset3
219268	9	420367	7	NULL	NULL	0	NULL	29.0 + / - 4.5 ml X 100 g-1 X min-1	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , at similar levels of hypocapnia ( PaCO2 18-20 mmHg ) , CBF was significantly lower ( P less than 0.01 ) during administration of isoflurane-N2O ( 29.0 + / - 4.5 ml X 100 g-1 X min-1 ) than during administration of either N2O ( 40.6 + / - 5.5 ml X 100 g-1 X min-1 ) or halothane-N2O ( 39.6 + / - 7.8 ml X 100 g-1 X min-1 ) .
	manualset3
219269	10	420367	7	NULL	NULL	0	NULL	administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , at similar levels of hypocapnia ( PaCO2 18-20 mmHg ) , CBF was significantly lower ( P less than 0.01 ) during administration of isoflurane-N2O ( 29.0 + / - 4.5 ml X 100 g-1 X min-1 ) than during administration of either N2O ( 40.6 + / - 5.5 ml X 100 g-1 X min-1 ) or halothane-N2O ( 39.6 + / - 7.8 ml X 100 g-1 X min-1 ) .
	manualset3
219270	11	420367	7	NULL	NULL	0	NULL	N2O	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , at similar levels of hypocapnia ( PaCO2 18-20 mmHg ) , CBF was significantly lower ( P less than 0.01 ) during administration of isoflurane-N2O ( 29.0 + / - 4.5 ml X 100 g-1 X min-1 ) than during administration of either N2O ( 40.6 + / - 5.5 ml X 100 g-1 X min-1 ) or halothane-N2O ( 39.6 + / - 7.8 ml X 100 g-1 X min-1 ) .
	manualset3
219271	12	420367	7	NULL	NULL	0	NULL	40.6 + / - 5.5 ml X 100 g-1 X min-1	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , at similar levels of hypocapnia ( PaCO2 18-20 mmHg ) , CBF was significantly lower ( P less than 0.01 ) during administration of isoflurane-N2O ( 29.0 + / - 4.5 ml X 100 g-1 X min-1 ) than during administration of either N2O ( 40.6 + / - 5.5 ml X 100 g-1 X min-1 ) or halothane-N2O ( 39.6 + / - 7.8 ml X 100 g-1 X min-1 ) .
	manualset3
219272	13	420367	7	NULL	NULL	0	NULL	halothane-N2O	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , at similar levels of hypocapnia ( PaCO2 18-20 mmHg ) , CBF was significantly lower ( P less than 0.01 ) during administration of isoflurane-N2O ( 29.0 + / - 4.5 ml X 100 g-1 X min-1 ) than during administration of either N2O ( 40.6 + / - 5.5 ml X 100 g-1 X min-1 ) or halothane-N2O ( 39.6 + / - 7.8 ml X 100 g-1 X min-1 ) .
	manualset3
219273	14	420367	7	NULL	NULL	0	NULL	39.6 + / - 7.8 ml X 100 g-1 X min-1 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , at similar levels of hypocapnia ( PaCO2 18-20 mmHg ) , CBF was significantly lower ( P less than 0.01 ) during administration of isoflurane-N2O ( 29.0 + / - 4.5 ml X 100 g-1 X min-1 ) than during administration of either N2O ( 40.6 + / - 5.5 ml X 100 g-1 X min-1 ) or halothane-N2O ( 39.6 + / - 7.8 ml X 100 g-1 X min-1 ) .
	manualset3
219274	1	420368	7	NULL	NULL	0	NULL	Strains 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains of Bacillus subtilis deficient in aspartokinases II and III are unable to grow in the absence of lysine , methionine , and threonine , although they have normal levels of aspartokinase I ( J.J. Zhang , F.M. Hu , N.Y. Chen , and H. Paulus , J. Bacteriol .
	manualset3
219275	2	420368	7	NULL	NULL	0	NULL	Bacillus subtilis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains of Bacillus subtilis deficient in aspartokinases II and III are unable to grow in the absence of lysine , methionine , and threonine , although they have normal levels of aspartokinase I ( J.J. Zhang , F.M. Hu , N.Y. Chen , and H. Paulus , J. Bacteriol .
	manualset3
219276	3	420368	7	NULL	NULL	0	NULL	aspartokinases II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains of Bacillus subtilis deficient in aspartokinases II and III are unable to grow in the absence of lysine , methionine , and threonine , although they have normal levels of aspartokinase I ( J.J. Zhang , F.M. Hu , N.Y. Chen , and H. Paulus , J. Bacteriol .
	manualset3
219277	4	420368	7	NULL	NULL	0	NULL	aspartokinases III	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains of Bacillus subtilis deficient in aspartokinases II and III are unable to grow in the absence of lysine , methionine , and threonine , although they have normal levels of aspartokinase I ( J.J. Zhang , F.M. Hu , N.Y. Chen , and H. Paulus , J. Bacteriol .
	manualset3
219278	5	420368	7	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains of Bacillus subtilis deficient in aspartokinases II and III are unable to grow in the absence of lysine , methionine , and threonine , although they have normal levels of aspartokinase I ( J.J. Zhang , F.M. Hu , N.Y. Chen , and H. Paulus , J. Bacteriol .
	manualset3
219279	6	420368	7	NULL	NULL	0	NULL	lysine 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains of Bacillus subtilis deficient in aspartokinases II and III are unable to grow in the absence of lysine , methionine , and threonine , although they have normal levels of aspartokinase I ( J.J. Zhang , F.M. Hu , N.Y. Chen , and H. Paulus , J. Bacteriol .
	manualset3
219280	7	420368	7	NULL	NULL	0	NULL	methionine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains of Bacillus subtilis deficient in aspartokinases II and III are unable to grow in the absence of lysine , methionine , and threonine , although they have normal levels of aspartokinase I ( J.J. Zhang , F.M. Hu , N.Y. Chen , and H. Paulus , J. Bacteriol .
	manualset3
219281	8	420368	7	NULL	NULL	0	NULL	threonine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains of Bacillus subtilis deficient in aspartokinases II and III are unable to grow in the absence of lysine , methionine , and threonine , although they have normal levels of aspartokinase I ( J.J. Zhang , F.M. Hu , N.Y. Chen , and H. Paulus , J. Bacteriol .
	manualset3
219282	9	420368	7	NULL	NULL	0	NULL	normal levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains of Bacillus subtilis deficient in aspartokinases II and III are unable to grow in the absence of lysine , methionine , and threonine , although they have normal levels of aspartokinase I ( J.J. Zhang , F.M. Hu , N.Y. Chen , and H. Paulus , J. Bacteriol .
	manualset3
219283	10	420368	7	NULL	NULL	0	NULL	aspartokinase I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains of Bacillus subtilis deficient in aspartokinases II and III are unable to grow in the absence of lysine , methionine , and threonine , although they have normal levels of aspartokinase I ( J.J. Zhang , F.M. Hu , N.Y. Chen , and H. Paulus , J. Bacteriol .
	manualset3
219284	11	420368	7	NULL	NULL	0	NULL	J.J. Zhang , F.M. Hu , N.Y. Chen , and H. Paulus , J. Bacteriol 	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	Strains of Bacillus subtilis deficient in aspartokinases II and III are unable to grow in the absence of lysine , methionine , and threonine , although they have normal levels of aspartokinase I ( J.J. Zhang , F.M. Hu , N.Y. Chen , and H. Paulus , J. Bacteriol .
	manualset3
219285	1	420369	7	NULL	NULL	0	NULL	 effort ,	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To support this effort , a matrix - ( seabird egg ) and concentration-specific control material was needed to ensure quality during analytical work .
	manualset3
219286	2	420369	7	NULL	NULL	0	NULL	matrix - ( seabird egg )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To support this effort , a matrix - ( seabird egg ) and concentration-specific control material was needed to ensure quality during analytical work .
	manualset3
219287	3	420369	7	NULL	NULL	0	NULL	concentration-specific control material	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	To support this effort , a matrix - ( seabird egg ) and concentration-specific control material was needed to ensure quality during analytical work .
	manualset3
219288	4	420369	7	NULL	NULL	0	NULL	quality	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To support this effort , a matrix - ( seabird egg ) and concentration-specific control material was needed to ensure quality during analytical work .
	manualset3
219289	5	420369	7	NULL	NULL	0	NULL	analytical work	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To support this effort , a matrix - ( seabird egg ) and concentration-specific control material was needed to ensure quality during analytical work .
	manualset3
219290	1	420370	7	NULL	NULL	0	NULL	 rat liver cytosol	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In rat liver cytosol at low concentrations , sulfobromophthalein bound to the 22 kDa subunit of ligandin .
	manualset3
219291	2	420370	7	NULL	NULL	0	NULL	low concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In rat liver cytosol at low concentrations , sulfobromophthalein bound to the 22 kDa subunit of ligandin .
	manualset3
219292	3	420370	7	NULL	NULL	0	NULL	sulfobromophthalein	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In rat liver cytosol at low concentrations , sulfobromophthalein bound to the 22 kDa subunit of ligandin .
	manualset3
219293	4	420370	7	NULL	NULL	0	NULL	22 kDa subunit	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In rat liver cytosol at low concentrations , sulfobromophthalein bound to the 22 kDa subunit of ligandin .
	manualset3
219294	5	420370	7	NULL	NULL	0	NULL	ligandin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In rat liver cytosol at low concentrations , sulfobromophthalein bound to the 22 kDa subunit of ligandin .
	manualset3
219401	1	420371	7	NULL	NULL	0	NULL	acetic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Replacing acetic acid with these dicarboxylic acids for membrane preparation improved the water uptake ( by 35 % at most ) , tensile strength ( by 110 % at most ) , and elongation capability ( by 50 % at most ) of the membranes .
	manualset3
219402	2	420371	7	NULL	NULL	0	NULL	dicarboxylic acids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Replacing acetic acid with these dicarboxylic acids for membrane preparation improved the water uptake ( by 35 % at most ) , tensile strength ( by 110 % at most ) , and elongation capability ( by 50 % at most ) of the membranes .
	manualset3
219403	3	420371	7	NULL	NULL	0	NULL	membrane preparation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Replacing acetic acid with these dicarboxylic acids for membrane preparation improved the water uptake ( by 35 % at most ) , tensile strength ( by 110 % at most ) , and elongation capability ( by 50 % at most ) of the membranes .
	manualset3
219404	4	420371	7	NULL	NULL	0	NULL	water uptake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Replacing acetic acid with these dicarboxylic acids for membrane preparation improved the water uptake ( by 35 % at most ) , tensile strength ( by 110 % at most ) , and elongation capability ( by 50 % at most ) of the membranes .
	manualset3
219405	5	420371	7	NULL	NULL	0	NULL	35 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Replacing acetic acid with these dicarboxylic acids for membrane preparation improved the water uptake ( by 35 % at most ) , tensile strength ( by 110 % at most ) , and elongation capability ( by 50 % at most ) of the membranes .
	manualset3
219406	6	420371	7	NULL	NULL	0	NULL	tensile strength	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Replacing acetic acid with these dicarboxylic acids for membrane preparation improved the water uptake ( by 35 % at most ) , tensile strength ( by 110 % at most ) , and elongation capability ( by 50 % at most ) of the membranes .
	manualset3
219407	7	420371	7	NULL	NULL	0	NULL	110 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Replacing acetic acid with these dicarboxylic acids for membrane preparation improved the water uptake ( by 35 % at most ) , tensile strength ( by 110 % at most ) , and elongation capability ( by 50 % at most ) of the membranes .
	manualset3
219408	8	420371	7	NULL	NULL	0	NULL	 elongation capability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Replacing acetic acid with these dicarboxylic acids for membrane preparation improved the water uptake ( by 35 % at most ) , tensile strength ( by 110 % at most ) , and elongation capability ( by 50 % at most ) of the membranes .
	manualset3
219409	9	420371	7	NULL	NULL	0	NULL	50 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Replacing acetic acid with these dicarboxylic acids for membrane preparation improved the water uptake ( by 35 % at most ) , tensile strength ( by 110 % at most ) , and elongation capability ( by 50 % at most ) of the membranes .
	manualset3
219410	10	420371	7	NULL	NULL	0	NULL	membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Replacing acetic acid with these dicarboxylic acids for membrane preparation improved the water uptake ( by 35 % at most ) , tensile strength ( by 110 % at most ) , and elongation capability ( by 50 % at most ) of the membranes .
	manualset3
219411	1	420372	7	NULL	NULL	0	NULL	incorporation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The incorporation of labeled chylomicrons into the fat emboli in the post-alimentary dog .
	manualset3
219412	2	420372	7	NULL	NULL	0	NULL	labeled chylomicrons	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The incorporation of labeled chylomicrons into the fat emboli in the post-alimentary dog .
	manualset3
219413	3	420372	7	NULL	NULL	0	NULL	fat emboli	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incorporation of labeled chylomicrons into the fat emboli in the post-alimentary dog .
	manualset3
219414	4	420372	7	NULL	NULL	0	NULL	post-alimentary dog	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The incorporation of labeled chylomicrons into the fat emboli in the post-alimentary dog .
	manualset3
219415	1	420373	7	NULL	NULL	0	NULL	Antibiotic resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic resistance , beta-lactamase activity , and plasmid content in strains of Haemophilus and Branhamella isolated from children .
	manualset3
219416	2	420373	7	NULL	NULL	NULL	NULL	beta-lactamase activity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Antibiotic resistance , beta-lactamase activity , and plasmid content in strains of Haemophilus and Branhamella isolated from children .
	manualset3
219417	3	420373	7	NULL	NULL	0	NULL	 plasmid content 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic resistance , beta-lactamase activity , and plasmid content in strains of Haemophilus and Branhamella isolated from children .
	manualset3
219418	4	420373	7	NULL	NULL	0	NULL	strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic resistance , beta-lactamase activity , and plasmid content in strains of Haemophilus and Branhamella isolated from children .
	manualset3
219419	5	420373	7	NULL	NULL	0	NULL	Haemophilus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic resistance , beta-lactamase activity , and plasmid content in strains of Haemophilus and Branhamella isolated from children .
	manualset3
219420	6	420373	7	NULL	NULL	0	NULL	Branhamella	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic resistance , beta-lactamase activity , and plasmid content in strains of Haemophilus and Branhamella isolated from children .
	manualset3
219421	7	420373	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic resistance , beta-lactamase activity , and plasmid content in strains of Haemophilus and Branhamella isolated from children .
	manualset3
219422	1	420374	7	NULL	NULL	0	NULL	noncovalent domino effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the importance of noncovalent domino effect for controlling the helical screw sense or helical stability of a chiral peptide has been demonstrated here for the first time .
	manualset3
219423	2	420374	7	NULL	NULL	0	NULL	helical screw sense	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the importance of noncovalent domino effect for controlling the helical screw sense or helical stability of a chiral peptide has been demonstrated here for the first time .
	manualset3
219424	3	420374	7	NULL	NULL	0	NULL	helical stability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the importance of noncovalent domino effect for controlling the helical screw sense or helical stability of a chiral peptide has been demonstrated here for the first time .
	manualset3
219425	4	420374	7	NULL	NULL	0	NULL	chiral peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the importance of noncovalent domino effect for controlling the helical screw sense or helical stability of a chiral peptide has been demonstrated here for the first time .
	manualset3
219426	5	420374	7	NULL	NULL	0	NULL	first time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , the importance of noncovalent domino effect for controlling the helical screw sense or helical stability of a chiral peptide has been demonstrated here for the first time .
	manualset3
219427	1	420375	7	NULL	NULL	0	NULL	Magnetic resonance ( MR ) images	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic resonance ( MR ) images of the brain showed multiple high-intensity spotty lesions in the left cerebral cortex and subcortex .
	manualset3
219428	2	420375	7	NULL	NULL	0	NULL	brain 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic resonance ( MR ) images of the brain showed multiple high-intensity spotty lesions in the left cerebral cortex and subcortex .
	manualset3
219429	3	420375	7	NULL	NULL	0	NULL	multiple high-intensity spotty lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic resonance ( MR ) images of the brain showed multiple high-intensity spotty lesions in the left cerebral cortex and subcortex .
	manualset3
219430	4	420375	7	NULL	NULL	0	NULL	left cerebral cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic resonance ( MR ) images of the brain showed multiple high-intensity spotty lesions in the left cerebral cortex and subcortex .
	manualset3
219431	5	420375	7	NULL	NULL	0	NULL	subcortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Magnetic resonance ( MR ) images of the brain showed multiple high-intensity spotty lesions in the left cerebral cortex and subcortex .
	manualset3
219432	1	420376	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , our studies shed more light on the role that adhesion molecules play within the neutrophil/NK cell/slanDC network .
	manualset3
219433	2	420376	7	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , our studies shed more light on the role that adhesion molecules play within the neutrophil/NK cell/slanDC network .
	manualset3
219434	3	420376	7	NULL	NULL	0	NULL	adhesion molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , our studies shed more light on the role that adhesion molecules play within the neutrophil/NK cell/slanDC network .
	manualset3
219435	4	420376	7	NULL	NULL	0	NULL	neutrophil/NK cell/slanDC network 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , our studies shed more light on the role that adhesion molecules play within the neutrophil/NK cell/slanDC network .
	manualset3
219436	1	420377	7	NULL	NULL	0	NULL	Uptake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Uptake of tritiated liquids by individual breakfast cereal flakes .
	manualset3
219437	2	420377	7	NULL	NULL	0	NULL	tritiated liquids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Uptake of tritiated liquids by individual breakfast cereal flakes .
	manualset3
219438	3	420377	7	NULL	NULL	0	NULL	individual breakfast cereal flakes	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Uptake of tritiated liquids by individual breakfast cereal flakes .
	manualset3
219439	1	420378	7	NULL	NULL	NULL	NULL	unusual features	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The unusual features in the proband that distinguish him from previously described cases and from his affected first-degree relatives suggested that , in addition to the basic gene defect affecting LDL metabolism , he might have a second abnormality affecting clearance of chylomicrons and VLDL .
	manualset3
219440	2	420378	7	NULL	NULL	0	NULL	proband	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The unusual features in the proband that distinguish him from previously described cases and from his affected first-degree relatives suggested that , in addition to the basic gene defect affecting LDL metabolism , he might have a second abnormality affecting clearance of chylomicrons and VLDL .
	manualset3
219441	3	420378	7	NULL	NULL	0	NULL	cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The unusual features in the proband that distinguish him from previously described cases and from his affected first-degree relatives suggested that , in addition to the basic gene defect affecting LDL metabolism , he might have a second abnormality affecting clearance of chylomicrons and VLDL .
	manualset3
219442	4	420378	7	NULL	NULL	0	NULL	affected first-degree relatives	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The unusual features in the proband that distinguish him from previously described cases and from his affected first-degree relatives suggested that , in addition to the basic gene defect affecting LDL metabolism , he might have a second abnormality affecting clearance of chylomicrons and VLDL .
	manualset3
219443	5	420378	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The unusual features in the proband that distinguish him from previously described cases and from his affected first-degree relatives suggested that , in addition to the basic gene defect affecting LDL metabolism , he might have a second abnormality affecting clearance of chylomicrons and VLDL .
	manualset3
219444	6	420378	7	NULL	NULL	0	NULL	basic gene defect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The unusual features in the proband that distinguish him from previously described cases and from his affected first-degree relatives suggested that , in addition to the basic gene defect affecting LDL metabolism , he might have a second abnormality affecting clearance of chylomicrons and VLDL .
	manualset3
219445	7	420378	7	NULL	NULL	0	NULL	LDL metabolism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The unusual features in the proband that distinguish him from previously described cases and from his affected first-degree relatives suggested that , in addition to the basic gene defect affecting LDL metabolism , he might have a second abnormality affecting clearance of chylomicrons and VLDL .
	manualset3
219446	8	420378	7	NULL	NULL	0	NULL	second abnormality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The unusual features in the proband that distinguish him from previously described cases and from his affected first-degree relatives suggested that , in addition to the basic gene defect affecting LDL metabolism , he might have a second abnormality affecting clearance of chylomicrons and VLDL .
	manualset3
219447	9	420378	7	NULL	NULL	0	NULL	clearance	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The unusual features in the proband that distinguish him from previously described cases and from his affected first-degree relatives suggested that , in addition to the basic gene defect affecting LDL metabolism , he might have a second abnormality affecting clearance of chylomicrons and VLDL .
	manualset3
219448	10	420378	7	NULL	NULL	0	NULL	chylomicrons	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The unusual features in the proband that distinguish him from previously described cases and from his affected first-degree relatives suggested that , in addition to the basic gene defect affecting LDL metabolism , he might have a second abnormality affecting clearance of chylomicrons and VLDL .
	manualset3
219449	11	420378	7	NULL	NULL	0	NULL	VLDL	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The unusual features in the proband that distinguish him from previously described cases and from his affected first-degree relatives suggested that , in addition to the basic gene defect affecting LDL metabolism , he might have a second abnormality affecting clearance of chylomicrons and VLDL .
	manualset3
219450	1	420379	7	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This review discusses our current understanding of histone acetyltransferases ( HATs ) or acetyltransferases ( ATs ) : their discovery , substrate specificity , catalytic mechanism , regulation , and functional links to transcription , as well as to other chromatin-modifying activities .
	manualset3
219451	2	420379	7	NULL	NULL	NULL	NULL	current understanding 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This review discusses our current understanding of histone acetyltransferases ( HATs ) or acetyltransferases ( ATs ) : their discovery , substrate specificity , catalytic mechanism , regulation , and functional links to transcription , as well as to other chromatin-modifying activities .
	manualset3
219452	3	420379	7	NULL	NULL	0	NULL	histone acetyltransferases ( HATs ) 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This review discusses our current understanding of histone acetyltransferases ( HATs ) or acetyltransferases ( ATs ) : their discovery , substrate specificity , catalytic mechanism , regulation , and functional links to transcription , as well as to other chromatin-modifying activities .
	manualset3
219453	4	420379	7	NULL	NULL	0	NULL	acetyltransferases ( ATs )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This review discusses our current understanding of histone acetyltransferases ( HATs ) or acetyltransferases ( ATs ) : their discovery , substrate specificity , catalytic mechanism , regulation , and functional links to transcription , as well as to other chromatin-modifying activities .
	manualset3
219454	5	420379	7	NULL	NULL	0	NULL	discovery	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This review discusses our current understanding of histone acetyltransferases ( HATs ) or acetyltransferases ( ATs ) : their discovery , substrate specificity , catalytic mechanism , regulation , and functional links to transcription , as well as to other chromatin-modifying activities .
	manualset3
219455	6	420379	7	NULL	NULL	NULL	NULL	substrate specificity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This review discusses our current understanding of histone acetyltransferases ( HATs ) or acetyltransferases ( ATs ) : their discovery , substrate specificity , catalytic mechanism , regulation , and functional links to transcription , as well as to other chromatin-modifying activities .
	manualset3
219456	7	420379	7	NULL	NULL	0	NULL	catalytic mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This review discusses our current understanding of histone acetyltransferases ( HATs ) or acetyltransferases ( ATs ) : their discovery , substrate specificity , catalytic mechanism , regulation , and functional links to transcription , as well as to other chromatin-modifying activities .
	manualset3
219457	8	420379	7	NULL	NULL	0	NULL	regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This review discusses our current understanding of histone acetyltransferases ( HATs ) or acetyltransferases ( ATs ) : their discovery , substrate specificity , catalytic mechanism , regulation , and functional links to transcription , as well as to other chromatin-modifying activities .
	manualset3
219458	9	420379	7	NULL	NULL	0	NULL	transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This review discusses our current understanding of histone acetyltransferases ( HATs ) or acetyltransferases ( ATs ) : their discovery , substrate specificity , catalytic mechanism , regulation , and functional links to transcription , as well as to other chromatin-modifying activities .
	manualset3
219459	10	420379	7	NULL	NULL	NULL	NULL	chromatin-modifying activities	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This review discusses our current understanding of histone acetyltransferases ( HATs ) or acetyltransferases ( ATs ) : their discovery , substrate specificity , catalytic mechanism , regulation , and functional links to transcription , as well as to other chromatin-modifying activities .
	manualset3
220507	11	420379	7	NULL	NULL	NULL	NULL	functional links	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This review discusses our current understanding of histone acetyltransferases ( HATs ) or acetyltransferases ( ATs ) : their discovery , substrate specificity , catalytic mechanism , regulation , and functional links to transcription , as well as to other chromatin-modifying activities .
	manualset3
219460	1	420380	7	NULL	NULL	0	NULL	Legal immunity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Legal immunity for the physician and hospital ) .
	manualset3
219461	2	420380	7	NULL	NULL	0	NULL	physician	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( Legal immunity for the physician and hospital ) .
	manualset3
219462	3	420380	7	NULL	NULL	0	NULL	hospital 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( Legal immunity for the physician and hospital ) .
	manualset3
219463	1	420381	7	NULL	NULL	0	NULL	 role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However the role APP plays in the adult retina and whether it is required for vision is unknown .
	manualset3
219464	2	420381	7	NULL	NULL	0	NULL	APP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However the role APP plays in the adult retina and whether it is required for vision is unknown .
	manualset3
219465	3	420381	7	NULL	NULL	0	NULL	adult retina	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However the role APP plays in the adult retina and whether it is required for vision is unknown .
	manualset3
219466	4	420381	7	NULL	NULL	0	NULL	vision	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However the role APP plays in the adult retina and whether it is required for vision is unknown .
	manualset3
219467	1	420382	7	NULL	NULL	0	NULL	proteomic approaches	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , both proteomic and in silico approaches identified more than 50 candidates for the as yet previously uncharacterized plastid envelope transporters .
	manualset3
219468	2	420382	7	NULL	NULL	0	NULL	in silico approaches	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , both proteomic and in silico approaches identified more than 50 candidates for the as yet previously uncharacterized plastid envelope transporters .
	manualset3
219469	3	420382	7	NULL	NULL	0	NULL	50 candidates	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , both proteomic and in silico approaches identified more than 50 candidates for the as yet previously uncharacterized plastid envelope transporters .
	manualset3
219470	4	420382	7	NULL	NULL	0	NULL	plastid envelope transporters	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , both proteomic and in silico approaches identified more than 50 candidates for the as yet previously uncharacterized plastid envelope transporters .
	manualset3
219471	1	420383	7	NULL	NULL	0	NULL	Diminished circadian organization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Diminished circadian organization in conjunction with the loss of cholinergic input to the cortex likely contributes to impaired cognition and behavior .
	manualset3
219472	2	420383	7	NULL	NULL	0	NULL	conjunction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Diminished circadian organization in conjunction with the loss of cholinergic input to the cortex likely contributes to impaired cognition and behavior .
	manualset3
219473	3	420383	7	NULL	NULL	0	NULL	loss	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Diminished circadian organization in conjunction with the loss of cholinergic input to the cortex likely contributes to impaired cognition and behavior .
	manualset3
219474	4	420383	7	NULL	NULL	0	NULL	cholinergic input 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Diminished circadian organization in conjunction with the loss of cholinergic input to the cortex likely contributes to impaired cognition and behavior .
	manualset3
219475	5	420383	7	NULL	NULL	0	NULL	cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Diminished circadian organization in conjunction with the loss of cholinergic input to the cortex likely contributes to impaired cognition and behavior .
	manualset3
219476	6	420383	7	NULL	NULL	0	NULL	impaired cognition 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Diminished circadian organization in conjunction with the loss of cholinergic input to the cortex likely contributes to impaired cognition and behavior .
	manualset3
219477	7	420383	7	NULL	NULL	0	NULL	behavior	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Diminished circadian organization in conjunction with the loss of cholinergic input to the cortex likely contributes to impaired cognition and behavior .
	manualset3
219478	1	420384	7	NULL	NULL	0	NULL	distinction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The distinction between scaphoid and fusiform megalourethra seems arbitrary , and the disorder is better viewed as a spectrum rather than as 2 distinct entities .
	manualset3
219479	2	420384	7	NULL	NULL	0	NULL	scaphoid megalourethra	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The distinction between scaphoid and fusiform megalourethra seems arbitrary , and the disorder is better viewed as a spectrum rather than as 2 distinct entities .
	manualset3
219480	3	420384	7	NULL	NULL	0	NULL	fusiform megalourethra	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The distinction between scaphoid and fusiform megalourethra seems arbitrary , and the disorder is better viewed as a spectrum rather than as 2 distinct entities .
	manualset3
219481	4	420384	7	NULL	NULL	0	NULL	disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The distinction between scaphoid and fusiform megalourethra seems arbitrary , and the disorder is better viewed as a spectrum rather than as 2 distinct entities .
	manualset3
219482	5	420384	7	NULL	NULL	0	NULL	spectrum	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The distinction between scaphoid and fusiform megalourethra seems arbitrary , and the disorder is better viewed as a spectrum rather than as 2 distinct entities .
	manualset3
219483	6	420384	7	NULL	NULL	0	NULL	2 distinct entities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The distinction between scaphoid and fusiform megalourethra seems arbitrary , and the disorder is better viewed as a spectrum rather than as 2 distinct entities .
	manualset3
219484	1	420385	7	NULL	NULL	0	NULL	Synthesis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Synthesis and activities of ring C oxygenated sterols .
	manualset3
219485	2	420385	7	NULL	NULL	0	NULL	activities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Synthesis and activities of ring C oxygenated sterols .
	manualset3
219486	3	420385	7	NULL	NULL	0	NULL	ring C oxygenated sterols	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Synthesis and activities of ring C oxygenated sterols .
	manualset3
219487	1	420386	7	NULL	NULL	0	NULL	Mass spectrometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mass spectrometry is well-suited for complex mixture analysis , because unlike other types of spectroscopy , the number of mass spectral peaks per analyte is of order one .
	manualset3
219488	2	420386	7	NULL	NULL	0	NULL	complex mixture analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mass spectrometry is well-suited for complex mixture analysis , because unlike other types of spectroscopy , the number of mass spectral peaks per analyte is of order one .
	manualset3
219489	3	420386	7	NULL	NULL	0	NULL	types of spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mass spectrometry is well-suited for complex mixture analysis , because unlike other types of spectroscopy , the number of mass spectral peaks per analyte is of order one .
	manualset3
219490	4	420386	7	NULL	NULL	0	NULL	 number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mass spectrometry is well-suited for complex mixture analysis , because unlike other types of spectroscopy , the number of mass spectral peaks per analyte is of order one .
	manualset3
219491	5	420386	7	NULL	NULL	0	NULL	mass spectral peaks per analyte	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mass spectrometry is well-suited for complex mixture analysis , because unlike other types of spectroscopy , the number of mass spectral peaks per analyte is of order one .
	manualset3
219492	6	420386	7	NULL	NULL	0	NULL	 order one 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mass spectrometry is well-suited for complex mixture analysis , because unlike other types of spectroscopy , the number of mass spectral peaks per analyte is of order one .
	manualset3
219539	1	420387	7	NULL	NULL	0	NULL	docking models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , the docking models support the proposal that the stabilization of a closed state represents a key step in agonist activation of mGluRs .
	manualset3
219540	2	420387	7	NULL	NULL	0	NULL	proposal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , the docking models support the proposal that the stabilization of a closed state represents a key step in agonist activation of mGluRs .
	manualset3
219541	3	420387	7	NULL	NULL	0	NULL	stabilization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , the docking models support the proposal that the stabilization of a closed state represents a key step in agonist activation of mGluRs .
	manualset3
219542	4	420387	7	NULL	NULL	0	NULL	closed state	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , the docking models support the proposal that the stabilization of a closed state represents a key step in agonist activation of mGluRs .
	manualset3
219543	5	420387	7	NULL	NULL	0	NULL	key step	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , the docking models support the proposal that the stabilization of a closed state represents a key step in agonist activation of mGluRs .
	manualset3
219544	6	420387	7	NULL	NULL	0	NULL	agonist activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , the docking models support the proposal that the stabilization of a closed state represents a key step in agonist activation of mGluRs .
	manualset3
219545	7	420387	7	NULL	NULL	0	NULL	mGluRs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , the docking models support the proposal that the stabilization of a closed state represents a key step in agonist activation of mGluRs .
	manualset3
219546	1	420388	7	NULL	NULL	0	NULL	Staphylococcal enterotoxin B ( SEB )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Staphylococcal enterotoxin B ( SEB ) is a common cause of food poisoning and toxic shock .
	manualset3
219547	2	420388	7	NULL	NULL	0	NULL	common cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Staphylococcal enterotoxin B ( SEB ) is a common cause of food poisoning and toxic shock .
	manualset3
219548	3	420388	7	NULL	NULL	0	NULL	food poisoning	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Staphylococcal enterotoxin B ( SEB ) is a common cause of food poisoning and toxic shock .
	manualset3
219549	4	420388	7	NULL	NULL	0	NULL	toxic shock	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Staphylococcal enterotoxin B ( SEB ) is a common cause of food poisoning and toxic shock .
	manualset3
219550	1	420389	7	NULL	NULL	0	NULL	Ghrelin levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ghrelin and obestatin levels in rheumatoid arthritis .
	manualset3
219551	2	420389	7	NULL	NULL	0	NULL	obestatin levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ghrelin and obestatin levels in rheumatoid arthritis .
	manualset3
219552	3	420389	7	NULL	NULL	0	NULL	rheumatoid arthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Ghrelin and obestatin levels in rheumatoid arthritis .
	manualset3
219553	1	420390	7	NULL	NULL	0	NULL	 immaturity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This immaturity involves all facets of respiration including respiratory responses to hypoxia , hypercapnia , an exaggerated apnoeic response to laryngeal stimulation and immature responses to activation of pulmonary afferents .
	manualset3
219554	2	420390	7	NULL	NULL	0	NULL	 facets of respiration 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This immaturity involves all facets of respiration including respiratory responses to hypoxia , hypercapnia , an exaggerated apnoeic response to laryngeal stimulation and immature responses to activation of pulmonary afferents .
	manualset3
219555	3	420390	7	NULL	NULL	0	NULL	respiratory responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This immaturity involves all facets of respiration including respiratory responses to hypoxia , hypercapnia , an exaggerated apnoeic response to laryngeal stimulation and immature responses to activation of pulmonary afferents .
	manualset3
219556	4	420390	7	NULL	NULL	0	NULL	hypoxia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This immaturity involves all facets of respiration including respiratory responses to hypoxia , hypercapnia , an exaggerated apnoeic response to laryngeal stimulation and immature responses to activation of pulmonary afferents .
	manualset3
219557	5	420390	7	NULL	NULL	0	NULL	hypercapnia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This immaturity involves all facets of respiration including respiratory responses to hypoxia , hypercapnia , an exaggerated apnoeic response to laryngeal stimulation and immature responses to activation of pulmonary afferents .
	manualset3
219558	6	420390	7	NULL	NULL	0	NULL	exaggerated apnoeic response 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This immaturity involves all facets of respiration including respiratory responses to hypoxia , hypercapnia , an exaggerated apnoeic response to laryngeal stimulation and immature responses to activation of pulmonary afferents .
	manualset3
219559	7	420390	7	NULL	NULL	0	NULL	laryngeal stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This immaturity involves all facets of respiration including respiratory responses to hypoxia , hypercapnia , an exaggerated apnoeic response to laryngeal stimulation and immature responses to activation of pulmonary afferents .
	manualset3
219560	8	420390	7	NULL	NULL	0	NULL	 immature responses 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This immaturity involves all facets of respiration including respiratory responses to hypoxia , hypercapnia , an exaggerated apnoeic response to laryngeal stimulation and immature responses to activation of pulmonary afferents .
	manualset3
219561	9	420390	7	NULL	NULL	0	NULL	activation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This immaturity involves all facets of respiration including respiratory responses to hypoxia , hypercapnia , an exaggerated apnoeic response to laryngeal stimulation and immature responses to activation of pulmonary afferents .
	manualset3
219562	10	420390	7	NULL	NULL	0	NULL	pulmonary afferents 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This immaturity involves all facets of respiration including respiratory responses to hypoxia , hypercapnia , an exaggerated apnoeic response to laryngeal stimulation and immature responses to activation of pulmonary afferents .
	manualset3
219563	1	420391	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitantly , the expression of pregnane X receptor ( PXR ) and constitutive androstane receptor ( CAR ) was diminished by COL , whereas expression of glucocorticoid receptor ( GR ) remained unaltered .
	manualset3
219564	2	420391	7	NULL	NULL	0	NULL	pregnane X receptor ( PXR ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitantly , the expression of pregnane X receptor ( PXR ) and constitutive androstane receptor ( CAR ) was diminished by COL , whereas expression of glucocorticoid receptor ( GR ) remained unaltered .
	manualset3
219565	3	420391	7	NULL	NULL	0	NULL	constitutive androstane receptor ( CAR )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitantly , the expression of pregnane X receptor ( PXR ) and constitutive androstane receptor ( CAR ) was diminished by COL , whereas expression of glucocorticoid receptor ( GR ) remained unaltered .
	manualset3
219566	4	420391	7	NULL	NULL	0	NULL	COL	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitantly , the expression of pregnane X receptor ( PXR ) and constitutive androstane receptor ( CAR ) was diminished by COL , whereas expression of glucocorticoid receptor ( GR ) remained unaltered .
	manualset3
219567	5	420391	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitantly , the expression of pregnane X receptor ( PXR ) and constitutive androstane receptor ( CAR ) was diminished by COL , whereas expression of glucocorticoid receptor ( GR ) remained unaltered .
	manualset3
219568	6	420391	7	NULL	NULL	0	NULL	glucocorticoid receptor ( GR ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitantly , the expression of pregnane X receptor ( PXR ) and constitutive androstane receptor ( CAR ) was diminished by COL , whereas expression of glucocorticoid receptor ( GR ) remained unaltered .
	manualset3
219569	1	420392	7	NULL	NULL	0	NULL	Regional localisation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Regional localisation of two non-specific X-linked mental retardation genes ( MRX30 and MRX31 ) .
	manualset3
219570	2	420392	7	NULL	NULL	0	NULL	two non-specific X-linked mental retardation genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Regional localisation of two non-specific X-linked mental retardation genes ( MRX30 and MRX31 ) .
	manualset3
219571	3	420392	7	NULL	NULL	0	NULL	MRX30	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Regional localisation of two non-specific X-linked mental retardation genes ( MRX30 and MRX31 ) .
	manualset3
219572	4	420392	7	NULL	NULL	0	NULL	MRX31	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Regional localisation of two non-specific X-linked mental retardation genes ( MRX30 and MRX31 ) .
	manualset3
219573	1	420393	7	NULL	NULL	0	NULL	Risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk of progression to active tuberculosis among foreign-born persons with latent tuberculosis .
	manualset3
219574	2	420393	7	NULL	NULL	0	NULL	progression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk of progression to active tuberculosis among foreign-born persons with latent tuberculosis .
	manualset3
219575	3	420393	7	NULL	NULL	0	NULL	active tuberculosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk of progression to active tuberculosis among foreign-born persons with latent tuberculosis .
	manualset3
219576	4	420393	7	NULL	NULL	0	NULL	foreign-born persons	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk of progression to active tuberculosis among foreign-born persons with latent tuberculosis .
	manualset3
219577	5	420393	7	NULL	NULL	0	NULL	latent tuberculosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Risk of progression to active tuberculosis among foreign-born persons with latent tuberculosis .
	manualset3
219578	1	420394	7	NULL	NULL	0	NULL	1 rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	1 rats , but a normal right-timed onset of puberty in both male and female rats .
	manualset3
219579	2	420394	7	NULL	NULL	0	NULL	 normal right-timed onset	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	1 rats , but a normal right-timed onset of puberty in both male and female rats .
	manualset3
219580	3	420394	7	NULL	NULL	0	NULL	puberty	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	1 rats , but a normal right-timed onset of puberty in both male and female rats .
	manualset3
219581	4	420394	7	NULL	NULL	0	NULL	male rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	1 rats , but a normal right-timed onset of puberty in both male and female rats .
	manualset3
219582	5	420394	7	NULL	NULL	0	NULL	female rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	1 rats , but a normal right-timed onset of puberty in both male and female rats .
	manualset3
219583	1	420395	7	NULL	NULL	0	NULL	four most significant peaks	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The four most significant peaks were selected out to train a genetic algorithm model to diagnose NPC .
	manualset3
219584	2	420395	7	NULL	NULL	0	NULL	genetic algorithm model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The four most significant peaks were selected out to train a genetic algorithm model to diagnose NPC .
	manualset3
219585	3	420395	7	NULL	NULL	0	NULL	NPC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The four most significant peaks were selected out to train a genetic algorithm model to diagnose NPC .
	manualset3
219586	1	420396	7	NULL	NULL	0	NULL	concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These same concentrations of forskolin reduced CAN currents reversibly to about 50 % .
	manualset3
219587	2	420396	7	NULL	NULL	0	NULL	forskolin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These same concentrations of forskolin reduced CAN currents reversibly to about 50 % .
	manualset3
219588	3	420396	7	NULL	NULL	0	NULL	CAN currents	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These same concentrations of forskolin reduced CAN currents reversibly to about 50 % .
	manualset3
219589	4	420396	7	NULL	NULL	0	NULL	50 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These same concentrations of forskolin reduced CAN currents reversibly to about 50 % .
	manualset3
219590	1	420397	7	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , the present study suggests a de-repression model and expands the understanding on the dynamic regulation of chromatin during myogenesis .
	manualset3
219591	2	420397	7	NULL	NULL	0	NULL	de-repression model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , the present study suggests a de-repression model and expands the understanding on the dynamic regulation of chromatin during myogenesis .
	manualset3
219592	3	420397	7	NULL	NULL	0	NULL	understanding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , the present study suggests a de-repression model and expands the understanding on the dynamic regulation of chromatin during myogenesis .
	manualset3
219593	4	420397	7	NULL	NULL	0	NULL	dynamic regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , the present study suggests a de-repression model and expands the understanding on the dynamic regulation of chromatin during myogenesis .
	manualset3
219594	5	420397	7	NULL	NULL	NULL	NULL	chromatin	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Altogether , the present study suggests a de-repression model and expands the understanding on the dynamic regulation of chromatin during myogenesis .
	manualset3
219595	6	420397	7	NULL	NULL	0	NULL	myogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , the present study suggests a de-repression model and expands the understanding on the dynamic regulation of chromatin during myogenesis .
	manualset3
219596	1	420398	7	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of type and dose of estrogen on the blood pressure of post-menopausal women .
	manualset3
219597	2	420398	7	NULL	NULL	0	NULL	type	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of type and dose of estrogen on the blood pressure of post-menopausal women .
	manualset3
219598	3	420398	7	NULL	NULL	0	NULL	dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of type and dose of estrogen on the blood pressure of post-menopausal women .
	manualset3
219599	4	420398	7	NULL	NULL	0	NULL	estrogen	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of type and dose of estrogen on the blood pressure of post-menopausal women .
	manualset3
219600	5	420398	7	NULL	NULL	0	NULL	blood pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of type and dose of estrogen on the blood pressure of post-menopausal women .
	manualset3
219601	6	420398	7	NULL	NULL	0	NULL	post-menopausal women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of type and dose of estrogen on the blood pressure of post-menopausal women .
	manualset3
219602	1	420399	7	NULL	NULL	0	NULL	PTZ	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	PTZ prolonged the membrane time constant by about 10 percent , but this could not be traced back to alterations in membrane resistance or capacity .
	manualset3
219603	2	420399	7	NULL	NULL	0	NULL	membrane time constant	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	PTZ prolonged the membrane time constant by about 10 percent , but this could not be traced back to alterations in membrane resistance or capacity .
	manualset3
219604	3	420399	7	NULL	NULL	0	NULL	10 percent	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PTZ prolonged the membrane time constant by about 10 percent , but this could not be traced back to alterations in membrane resistance or capacity .
	manualset3
219605	4	420399	7	NULL	NULL	0	NULL	alterations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PTZ prolonged the membrane time constant by about 10 percent , but this could not be traced back to alterations in membrane resistance or capacity .
	manualset3
219606	5	420399	7	NULL	NULL	0	NULL	membrane resistance	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PTZ prolonged the membrane time constant by about 10 percent , but this could not be traced back to alterations in membrane resistance or capacity .
	manualset3
219607	6	420399	7	NULL	NULL	0	NULL	membrane capacity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	PTZ prolonged the membrane time constant by about 10 percent , but this could not be traced back to alterations in membrane resistance or capacity .
	manualset3
219608	1	420400	7	NULL	NULL	0	NULL	Temperature-activity curves	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Temperature-activity curves were determined for asclepain on hemoglobin , casein , and milk solutions .
	manualset3
219609	2	420400	7	NULL	NULL	0	NULL	asclepain	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Temperature-activity curves were determined for asclepain on hemoglobin , casein , and milk solutions .
	manualset3
219610	3	420400	7	NULL	NULL	0	NULL	hemoglobin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Temperature-activity curves were determined for asclepain on hemoglobin , casein , and milk solutions .
	manualset3
219611	4	420400	7	NULL	NULL	0	NULL	casein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Temperature-activity curves were determined for asclepain on hemoglobin , casein , and milk solutions .
	manualset3
219612	5	420400	7	NULL	NULL	0	NULL	milk solutions 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Temperature-activity curves were determined for asclepain on hemoglobin , casein , and milk solutions .
	manualset3
219613	1	420401	7	NULL	NULL	0	NULL	Cecal volvulus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Cecal volvulus : report of seven cases and literature review .
	manualset3
219614	2	420401	7	NULL	NULL	0	NULL	 report 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Cecal volvulus : report of seven cases and literature review .
	manualset3
219615	3	420401	7	NULL	NULL	0	NULL	seven cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Cecal volvulus : report of seven cases and literature review .
	manualset3
219616	4	420401	7	NULL	NULL	0	NULL	literature review 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Cecal volvulus : report of seven cases and literature review .
	manualset3
219617	1	420402	7	NULL	NULL	0	NULL	Chronic lymphocytic leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic lymphocytic leukemia of the orbit .
	manualset3
219618	2	420402	7	NULL	NULL	0	NULL	orbit	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic lymphocytic leukemia of the orbit .
	manualset3
219619	1	420403	7	NULL	NULL	0	NULL	Intra uterine asphyxia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intra uterine asphyxia as a main factor of stillbirth ) .
	manualset3
219620	2	420403	7	NULL	NULL	0	NULL	main factor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intra uterine asphyxia as a main factor of stillbirth ) .
	manualset3
219621	3	420403	7	NULL	NULL	0	NULL	stillbirth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intra uterine asphyxia as a main factor of stillbirth ) .
	manualset3
219622	1	420404	7	NULL	NULL	0	NULL	Human limbal stem cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Human limbal stem cells produce transit amplifying progenitors that migrate centripetally to regenerate the corneal epithelium .
	manualset3
219623	2	420404	7	NULL	NULL	0	NULL	 transit amplifying progenitors	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Human limbal stem cells produce transit amplifying progenitors that migrate centripetally to regenerate the corneal epithelium .
	manualset3
219624	3	420404	7	NULL	NULL	0	NULL	corneal epithelium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Human limbal stem cells produce transit amplifying progenitors that migrate centripetally to regenerate the corneal epithelium .
	manualset3
219625	1	420405	7	NULL	NULL	0	NULL	Puncture	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Puncture of the internal jugular vein as an access for extracorporeal circulation in hemodialysis , hemoperfusion and plasma separation ) .
	manualset3
219626	2	420405	7	NULL	NULL	0	NULL	internal jugular vein	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Puncture of the internal jugular vein as an access for extracorporeal circulation in hemodialysis , hemoperfusion and plasma separation ) .
	manualset3
219627	3	420405	7	NULL	NULL	0	NULL	extracorporeal circulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Puncture of the internal jugular vein as an access for extracorporeal circulation in hemodialysis , hemoperfusion and plasma separation ) .
	manualset3
219628	4	420405	7	NULL	NULL	0	NULL	hemodialysis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Puncture of the internal jugular vein as an access for extracorporeal circulation in hemodialysis , hemoperfusion and plasma separation ) .
	manualset3
219629	5	420405	7	NULL	NULL	0	NULL	hemoperfusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Puncture of the internal jugular vein as an access for extracorporeal circulation in hemodialysis , hemoperfusion and plasma separation ) .
	manualset3
219630	6	420405	7	NULL	NULL	0	NULL	plasma separation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Puncture of the internal jugular vein as an access for extracorporeal circulation in hemodialysis , hemoperfusion and plasma separation ) .
	manualset3
219631	1	420406	7	NULL	NULL	0	NULL	Perioperative RNs	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Perioperative RNs should consider using red rules or a code of conduct as tools for improving the manual counting process .
	manualset3
219632	2	420406	7	NULL	NULL	0	NULL	 red rules 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Perioperative RNs should consider using red rules or a code of conduct as tools for improving the manual counting process .
	manualset3
219633	3	420406	7	NULL	NULL	0	NULL	code of conduct	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Perioperative RNs should consider using red rules or a code of conduct as tools for improving the manual counting process .
	manualset3
219634	4	420406	7	NULL	NULL	0	NULL	tools	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Perioperative RNs should consider using red rules or a code of conduct as tools for improving the manual counting process .
	manualset3
219635	5	420406	7	NULL	NULL	0	NULL	manual counting process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Perioperative RNs should consider using red rules or a code of conduct as tools for improving the manual counting process .
	manualset3
219636	1	420407	7	NULL	NULL	0	NULL	S487L change	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The S487L change is the predominant change found in rpoB mutations sequenced from rifampin-resistant clinical isolates of Mycobacterium tuberculosis .
	manualset3
219637	2	420407	7	NULL	NULL	0	NULL	change	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The S487L change is the predominant change found in rpoB mutations sequenced from rifampin-resistant clinical isolates of Mycobacterium tuberculosis .
	manualset3
219638	3	420407	7	NULL	NULL	0	NULL	rpoB mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The S487L change is the predominant change found in rpoB mutations sequenced from rifampin-resistant clinical isolates of Mycobacterium tuberculosis .
	manualset3
219639	4	420407	7	NULL	NULL	0	NULL	rifampin-resistant clinical isolates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The S487L change is the predominant change found in rpoB mutations sequenced from rifampin-resistant clinical isolates of Mycobacterium tuberculosis .
	manualset3
219640	5	420407	7	NULL	NULL	0	NULL	Mycobacterium tuberculosis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The S487L change is the predominant change found in rpoB mutations sequenced from rifampin-resistant clinical isolates of Mycobacterium tuberculosis .
	manualset3
219641	1	420408	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , these data indicate that HVA auxiliary subunits modulate Ca ( V ) 3 channel surface expression , suggesting that the membrane targeting of HVA and LVA alpha ( 1 ) subunits is regulated dynamically through the expression of a common set of regulatory subunits .
	manualset3
219642	2	420408	7	NULL	NULL	0	NULL	HVA auxiliary subunits	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , these data indicate that HVA auxiliary subunits modulate Ca ( V ) 3 channel surface expression , suggesting that the membrane targeting of HVA and LVA alpha ( 1 ) subunits is regulated dynamically through the expression of a common set of regulatory subunits .
	manualset3
219643	3	420408	7	NULL	NULL	0	NULL	Ca ( V ) 3 channel surface expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , these data indicate that HVA auxiliary subunits modulate Ca ( V ) 3 channel surface expression , suggesting that the membrane targeting of HVA and LVA alpha ( 1 ) subunits is regulated dynamically through the expression of a common set of regulatory subunits .
	manualset3
219644	4	420408	7	NULL	NULL	0	NULL	 membrane targeting	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , these data indicate that HVA auxiliary subunits modulate Ca ( V ) 3 channel surface expression , suggesting that the membrane targeting of HVA and LVA alpha ( 1 ) subunits is regulated dynamically through the expression of a common set of regulatory subunits .
	manualset3
219645	5	420408	7	NULL	NULL	0	NULL	HVA alpha subunits	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , these data indicate that HVA auxiliary subunits modulate Ca ( V ) 3 channel surface expression , suggesting that the membrane targeting of HVA and LVA alpha ( 1 ) subunits is regulated dynamically through the expression of a common set of regulatory subunits .
	manualset3
219646	6	420408	7	NULL	NULL	0	NULL	LVA alpha ( 1 ) subunits	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , these data indicate that HVA auxiliary subunits modulate Ca ( V ) 3 channel surface expression , suggesting that the membrane targeting of HVA and LVA alpha ( 1 ) subunits is regulated dynamically through the expression of a common set of regulatory subunits .
	manualset3
219647	7	420408	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , these data indicate that HVA auxiliary subunits modulate Ca ( V ) 3 channel surface expression , suggesting that the membrane targeting of HVA and LVA alpha ( 1 ) subunits is regulated dynamically through the expression of a common set of regulatory subunits .
	manualset3
219648	8	420408	7	NULL	NULL	0	NULL	common set	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , these data indicate that HVA auxiliary subunits modulate Ca ( V ) 3 channel surface expression , suggesting that the membrane targeting of HVA and LVA alpha ( 1 ) subunits is regulated dynamically through the expression of a common set of regulatory subunits .
	manualset3
219649	9	420408	7	NULL	NULL	0	NULL	regulatory subunits	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , these data indicate that HVA auxiliary subunits modulate Ca ( V ) 3 channel surface expression , suggesting that the membrane targeting of HVA and LVA alpha ( 1 ) subunits is regulated dynamically through the expression of a common set of regulatory subunits .
	manualset3
219650	1	420409	7	NULL	NULL	0	NULL	The jejunal tube	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( The jejunal tube : a possibility for early postoperative enteral feeding ) .
	manualset3
219651	2	420409	7	NULL	NULL	0	NULL	possibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The jejunal tube : a possibility for early postoperative enteral feeding ) .
	manualset3
219652	3	420409	7	NULL	NULL	NULL	NULL	early postoperative enteral feeding	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The jejunal tube : a possibility for early postoperative enteral feeding ) .
	manualset3
219653	1	420410	7	NULL	NULL	0	NULL	Biomechanics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Biomechanics of the human anterior cruciate ligament .
	manualset3
219654	2	420410	7	NULL	NULL	0	NULL	human anterior cruciate ligament 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Biomechanics of the human anterior cruciate ligament .
	manualset3
219655	1	420411	7	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	It is observed that the time required to complete the growth process for magnetite nanocrystals is very short ( approximately 300 s ) , compared to long digestion times ( 20-190 min ) required for MnO and CdSe nanocrystals .
	manualset3
219656	2	420411	7	NULL	NULL	0	NULL	growth process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is observed that the time required to complete the growth process for magnetite nanocrystals is very short ( approximately 300 s ) , compared to long digestion times ( 20-190 min ) required for MnO and CdSe nanocrystals .
	manualset3
219657	3	420411	7	NULL	NULL	0	NULL	magnetite nanocrystals	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	It is observed that the time required to complete the growth process for magnetite nanocrystals is very short ( approximately 300 s ) , compared to long digestion times ( 20-190 min ) required for MnO and CdSe nanocrystals .
	manualset3
219658	4	420411	7	NULL	NULL	0	NULL	300 s 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	It is observed that the time required to complete the growth process for magnetite nanocrystals is very short ( approximately 300 s ) , compared to long digestion times ( 20-190 min ) required for MnO and CdSe nanocrystals .
	manualset3
219659	5	420411	7	NULL	NULL	0	NULL	long digestion times	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	It is observed that the time required to complete the growth process for magnetite nanocrystals is very short ( approximately 300 s ) , compared to long digestion times ( 20-190 min ) required for MnO and CdSe nanocrystals .
	manualset3
219660	6	420411	7	NULL	NULL	0	NULL	20-190 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	It is observed that the time required to complete the growth process for magnetite nanocrystals is very short ( approximately 300 s ) , compared to long digestion times ( 20-190 min ) required for MnO and CdSe nanocrystals .
	manualset3
219661	7	420411	7	NULL	NULL	0	NULL	MnO nanocrystals	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	It is observed that the time required to complete the growth process for magnetite nanocrystals is very short ( approximately 300 s ) , compared to long digestion times ( 20-190 min ) required for MnO and CdSe nanocrystals .
	manualset3
219662	8	420411	7	NULL	NULL	0	NULL	CdSe nanocrystals	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	It is observed that the time required to complete the growth process for magnetite nanocrystals is very short ( approximately 300 s ) , compared to long digestion times ( 20-190 min ) required for MnO and CdSe nanocrystals .
	manualset3
219663	1	420412	7	NULL	NULL	0	NULL	Remodeling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Remodeling of human myocardial collagen in idiopathic dilated cardiomyopathy .
	manualset3
219664	2	420412	7	NULL	NULL	0	NULL	human myocardial collagen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Remodeling of human myocardial collagen in idiopathic dilated cardiomyopathy .
	manualset3
219665	3	420412	7	NULL	NULL	0	NULL	idiopathic dilated cardiomyopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Remodeling of human myocardial collagen in idiopathic dilated cardiomyopathy .
	manualset3
219666	1	420413	7	NULL	NULL	0	NULL	Overexpression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of ERRalpha significantly increased aromatase expression and promoter activity , which were further augmented by PGE2 .
	manualset3
219667	2	420413	7	NULL	NULL	0	NULL	ERRalpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of ERRalpha significantly increased aromatase expression and promoter activity , which were further augmented by PGE2 .
	manualset3
219668	3	420413	7	NULL	NULL	0	NULL	aromatase expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of ERRalpha significantly increased aromatase expression and promoter activity , which were further augmented by PGE2 .
	manualset3
219669	4	420413	7	NULL	NULL	0	NULL	promoter activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overexpression of ERRalpha significantly increased aromatase expression and promoter activity , which were further augmented by PGE2 .
	manualset3
219670	5	420413	7	NULL	NULL	NULL	NULL	PGE2	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Overexpression of ERRalpha significantly increased aromatase expression and promoter activity , which were further augmented by PGE2 .
	manualset3
219671	1	420414	7	NULL	NULL	0	NULL	Single-genome sequencing analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-genome sequencing analyses of the selected virus revealed a complex population of mutants that all contained L74V and L214F linked to other mutations , including ones not identified during population sequencing .
	manualset3
219672	2	420414	7	NULL	NULL	0	NULL	selected virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-genome sequencing analyses of the selected virus revealed a complex population of mutants that all contained L74V and L214F linked to other mutations , including ones not identified during population sequencing .
	manualset3
219673	3	420414	7	NULL	NULL	0	NULL	complex population	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-genome sequencing analyses of the selected virus revealed a complex population of mutants that all contained L74V and L214F linked to other mutations , including ones not identified during population sequencing .
	manualset3
219674	4	420414	7	NULL	NULL	0	NULL	mutants	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-genome sequencing analyses of the selected virus revealed a complex population of mutants that all contained L74V and L214F linked to other mutations , including ones not identified during population sequencing .
	manualset3
219675	5	420414	7	NULL	NULL	0	NULL	L74V	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-genome sequencing analyses of the selected virus revealed a complex population of mutants that all contained L74V and L214F linked to other mutations , including ones not identified during population sequencing .
	manualset3
219676	6	420414	7	NULL	NULL	0	NULL	L214F	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-genome sequencing analyses of the selected virus revealed a complex population of mutants that all contained L74V and L214F linked to other mutations , including ones not identified during population sequencing .
	manualset3
219677	7	420414	7	NULL	NULL	0	NULL	mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-genome sequencing analyses of the selected virus revealed a complex population of mutants that all contained L74V and L214F linked to other mutations , including ones not identified during population sequencing .
	manualset3
219678	8	420414	7	NULL	NULL	0	NULL	population sequencing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Single-genome sequencing analyses of the selected virus revealed a complex population of mutants that all contained L74V and L214F linked to other mutations , including ones not identified during population sequencing .
	manualset3
219679	1	420415	7	NULL	NULL	0	NULL	main factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The main factors determining the degree of O2 equilibration of gill water are shown to be interlamellar distance , length of the secondary lamellas , water velocity , and diffusion coefficient of O2 in water .
	manualset3
219680	2	420415	7	NULL	NULL	0	NULL	degree	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The main factors determining the degree of O2 equilibration of gill water are shown to be interlamellar distance , length of the secondary lamellas , water velocity , and diffusion coefficient of O2 in water .
	manualset3
219681	3	420415	7	NULL	NULL	NULL	NULL	O2 equilibration	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The main factors determining the degree of O2 equilibration of gill water are shown to be interlamellar distance , length of the secondary lamellas , water velocity , and diffusion coefficient of O2 in water .
	manualset3
219682	4	420415	7	NULL	NULL	NULL	NULL	gill water	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The main factors determining the degree of O2 equilibration of gill water are shown to be interlamellar distance , length of the secondary lamellas , water velocity , and diffusion coefficient of O2 in water .
	manualset3
219683	5	420415	7	NULL	NULL	0	NULL	interlamellar distance	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The main factors determining the degree of O2 equilibration of gill water are shown to be interlamellar distance , length of the secondary lamellas , water velocity , and diffusion coefficient of O2 in water .
	manualset3
219684	6	420415	7	NULL	NULL	NULL	NULL	 length 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The main factors determining the degree of O2 equilibration of gill water are shown to be interlamellar distance , length of the secondary lamellas , water velocity , and diffusion coefficient of O2 in water .
	manualset3
219685	7	420415	7	NULL	NULL	0	NULL	water velocity 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The main factors determining the degree of O2 equilibration of gill water are shown to be interlamellar distance , length of the secondary lamellas , water velocity , and diffusion coefficient of O2 in water .
	manualset3
219686	8	420415	7	NULL	NULL	0	NULL	diffusion coefficient	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The main factors determining the degree of O2 equilibration of gill water are shown to be interlamellar distance , length of the secondary lamellas , water velocity , and diffusion coefficient of O2 in water .
	manualset3
219687	9	420415	7	NULL	NULL	0	NULL	O2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The main factors determining the degree of O2 equilibration of gill water are shown to be interlamellar distance , length of the secondary lamellas , water velocity , and diffusion coefficient of O2 in water .
	manualset3
219688	10	420415	7	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The main factors determining the degree of O2 equilibration of gill water are shown to be interlamellar distance , length of the secondary lamellas , water velocity , and diffusion coefficient of O2 in water .
	manualset3
219689	11	420415	7	NULL	NULL	0	NULL	secondary lamellas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The main factors determining the degree of O2 equilibration of gill water are shown to be interlamellar distance , length of the secondary lamellas , water velocity , and diffusion coefficient of O2 in water .
	manualset3
219690	1	420416	7	NULL	NULL	0	NULL	Prospective evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prospective evaluation of a new high-power argon plasma coagulation system ( hp-APC ) in therapeutic gastrointestinal endoscopy .
	manualset3
219691	2	420416	7	NULL	NULL	0	NULL	new high-power argon plasma coagulation system ( hp-APC )	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Prospective evaluation of a new high-power argon plasma coagulation system ( hp-APC ) in therapeutic gastrointestinal endoscopy .
	manualset3
219692	3	420416	7	NULL	NULL	0	NULL	therapeutic gastrointestinal endoscopy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prospective evaluation of a new high-power argon plasma coagulation system ( hp-APC ) in therapeutic gastrointestinal endoscopy .
	manualset3
219693	1	420417	7	NULL	NULL	0	NULL	Deep brain stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Deep brain stimulation of the Vim nucleus of the thalamus in the treatment of parkinsonian tremor ) .
	manualset3
219694	2	420417	7	NULL	NULL	0	NULL	Vim nucleus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Deep brain stimulation of the Vim nucleus of the thalamus in the treatment of parkinsonian tremor ) .
	manualset3
219695	3	420417	7	NULL	NULL	0	NULL	thalamus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Deep brain stimulation of the Vim nucleus of the thalamus in the treatment of parkinsonian tremor ) .
	manualset3
219696	4	420417	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Deep brain stimulation of the Vim nucleus of the thalamus in the treatment of parkinsonian tremor ) .
	manualset3
219697	5	420417	7	NULL	NULL	0	NULL	parkinsonian tremor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Deep brain stimulation of the Vim nucleus of the thalamus in the treatment of parkinsonian tremor ) .
	manualset3
219698	1	420418	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , these results provide novel insights into the functional role of tau protein in the formation of collective neural responses and emergence of neocortical-hippocampal interactions in the mammalian brain .
	manualset3
219699	2	420418	7	NULL	NULL	0	NULL	functional role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , these results provide novel insights into the functional role of tau protein in the formation of collective neural responses and emergence of neocortical-hippocampal interactions in the mammalian brain .
	manualset3
219700	3	420418	7	NULL	NULL	0	NULL	tau protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , these results provide novel insights into the functional role of tau protein in the formation of collective neural responses and emergence of neocortical-hippocampal interactions in the mammalian brain .
	manualset3
219701	4	420418	7	NULL	NULL	0	NULL	formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , these results provide novel insights into the functional role of tau protein in the formation of collective neural responses and emergence of neocortical-hippocampal interactions in the mammalian brain .
	manualset3
219702	5	420418	7	NULL	NULL	0	NULL	collective neural responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , these results provide novel insights into the functional role of tau protein in the formation of collective neural responses and emergence of neocortical-hippocampal interactions in the mammalian brain .
	manualset3
219703	6	420418	7	NULL	NULL	0	NULL	emergence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , these results provide novel insights into the functional role of tau protein in the formation of collective neural responses and emergence of neocortical-hippocampal interactions in the mammalian brain .
	manualset3
219704	7	420418	7	NULL	NULL	0	NULL	neocortical-hippocampal interactions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , these results provide novel insights into the functional role of tau protein in the formation of collective neural responses and emergence of neocortical-hippocampal interactions in the mammalian brain .
	manualset3
219705	8	420418	7	NULL	NULL	0	NULL	mammalian brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , these results provide novel insights into the functional role of tau protein in the formation of collective neural responses and emergence of neocortical-hippocampal interactions in the mammalian brain .
	manualset3
219706	1	420419	7	NULL	NULL	0	NULL	Changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Changes in the plastic properties of the neuron under the action of antibodies to specific glycolipid antigens of the glia ) .
	manualset3
219707	2	420419	7	NULL	NULL	0	NULL	 plastic properties	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Changes in the plastic properties of the neuron under the action of antibodies to specific glycolipid antigens of the glia ) .
	manualset3
219708	3	420419	7	NULL	NULL	0	NULL	neuron	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Changes in the plastic properties of the neuron under the action of antibodies to specific glycolipid antigens of the glia ) .
	manualset3
219709	4	420419	7	NULL	NULL	0	NULL	action 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Changes in the plastic properties of the neuron under the action of antibodies to specific glycolipid antigens of the glia ) .
	manualset3
219710	5	420419	7	NULL	NULL	0	NULL	antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Changes in the plastic properties of the neuron under the action of antibodies to specific glycolipid antigens of the glia ) .
	manualset3
219711	6	420419	7	NULL	NULL	0	NULL	specific glycolipid antigens	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Changes in the plastic properties of the neuron under the action of antibodies to specific glycolipid antigens of the glia ) .
	manualset3
219712	7	420419	7	NULL	NULL	0	NULL	glia	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Changes in the plastic properties of the neuron under the action of antibodies to specific glycolipid antigens of the glia ) .
	manualset3
219713	1	420420	7	NULL	NULL	0	NULL	spontaneous porto-systemic shunts	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Even spontaneous porto-systemic shunts can be demonstrated in most cases ( up to 88 % ) .
	manualset3
219714	2	420420	7	NULL	NULL	0	NULL	cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Even spontaneous porto-systemic shunts can be demonstrated in most cases ( up to 88 % ) .
	manualset3
219715	3	420420	7	NULL	NULL	0	NULL	88 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Even spontaneous porto-systemic shunts can be demonstrated in most cases ( up to 88 % ) .
	manualset3
219716	1	420421	7	NULL	NULL	0	NULL	 majority	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , ultimately , the majority of diabetics will die from macrovascular cardiovascular disease .
	manualset3
219717	2	420421	7	NULL	NULL	0	NULL	diabetics	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , ultimately , the majority of diabetics will die from macrovascular cardiovascular disease .
	manualset3
219718	3	420421	7	NULL	NULL	0	NULL	macrovascular cardiovascular disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	However , ultimately , the majority of diabetics will die from macrovascular cardiovascular disease .
	manualset3
219719	1	420422	7	NULL	NULL	0	NULL	 frequencies	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequencies of this haplotype were 0.38 and 0.27 , respectively ( P = 0.0266 , chi2 ) .
	manualset3
219720	2	420422	7	NULL	NULL	0	NULL	haplotype	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequencies of this haplotype were 0.38 and 0.27 , respectively ( P = 0.0266 , chi2 ) .
	manualset3
219721	3	420422	7	NULL	NULL	0	NULL	0.38	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequencies of this haplotype were 0.38 and 0.27 , respectively ( P = 0.0266 , chi2 ) .
	manualset3
219722	4	420422	7	NULL	NULL	0	NULL	0.27	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequencies of this haplotype were 0.38 and 0.27 , respectively ( P = 0.0266 , chi2 ) .
	manualset3
219723	5	420422	7	NULL	NULL	0	NULL	P = 0.0266	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequencies of this haplotype were 0.38 and 0.27 , respectively ( P = 0.0266 , chi2 ) .
	manualset3
219724	6	420422	7	NULL	NULL	0	NULL	chi2	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequencies of this haplotype were 0.38 and 0.27 , respectively ( P = 0.0266 , chi2 ) .
	manualset3
219725	1	420423	7	NULL	NULL	0	NULL	Kinetic studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Kinetic studies of the induction of DNA synthesis by CTGF in cells arrested by cAMP indicate that the block occurs in very late G1 .
	manualset3
219726	2	420423	7	NULL	NULL	0	NULL	induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Kinetic studies of the induction of DNA synthesis by CTGF in cells arrested by cAMP indicate that the block occurs in very late G1 .
	manualset3
219727	3	420423	7	NULL	NULL	0	NULL	DNA synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Kinetic studies of the induction of DNA synthesis by CTGF in cells arrested by cAMP indicate that the block occurs in very late G1 .
	manualset3
219728	4	420423	7	NULL	NULL	0	NULL	CTGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Kinetic studies of the induction of DNA synthesis by CTGF in cells arrested by cAMP indicate that the block occurs in very late G1 .
	manualset3
219729	5	420423	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Kinetic studies of the induction of DNA synthesis by CTGF in cells arrested by cAMP indicate that the block occurs in very late G1 .
	manualset3
219730	6	420423	7	NULL	NULL	0	NULL	cAMP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Kinetic studies of the induction of DNA synthesis by CTGF in cells arrested by cAMP indicate that the block occurs in very late G1 .
	manualset3
219731	7	420423	7	NULL	NULL	NULL	NULL	block	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Kinetic studies of the induction of DNA synthesis by CTGF in cells arrested by cAMP indicate that the block occurs in very late G1 .
	manualset3
219732	8	420423	7	NULL	NULL	0	NULL	very late G1	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Kinetic studies of the induction of DNA synthesis by CTGF in cells arrested by cAMP indicate that the block occurs in very late G1 .
	manualset3
219733	1	420424	7	NULL	NULL	0	NULL	Background	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Background : Opioid-induced constipation can cause great discomfort to patients who use opioids for prolonged periods and on occasion decline pain-relief in an effort to help aid laxation .
	manualset3
219734	2	420424	7	NULL	NULL	0	NULL	Opioid-induced constipation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Background : Opioid-induced constipation can cause great discomfort to patients who use opioids for prolonged periods and on occasion decline pain-relief in an effort to help aid laxation .
	manualset3
219735	3	420424	7	NULL	NULL	0	NULL	discomfort 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Background : Opioid-induced constipation can cause great discomfort to patients who use opioids for prolonged periods and on occasion decline pain-relief in an effort to help aid laxation .
	manualset3
219736	4	420424	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Background : Opioid-induced constipation can cause great discomfort to patients who use opioids for prolonged periods and on occasion decline pain-relief in an effort to help aid laxation .
	manualset3
219737	5	420424	7	NULL	NULL	0	NULL	 opioids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Background : Opioid-induced constipation can cause great discomfort to patients who use opioids for prolonged periods and on occasion decline pain-relief in an effort to help aid laxation .
	manualset3
219738	6	420424	7	NULL	NULL	0	NULL	occasion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Background : Opioid-induced constipation can cause great discomfort to patients who use opioids for prolonged periods and on occasion decline pain-relief in an effort to help aid laxation .
	manualset3
219739	7	420424	7	NULL	NULL	0	NULL	pain-relief	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Background : Opioid-induced constipation can cause great discomfort to patients who use opioids for prolonged periods and on occasion decline pain-relief in an effort to help aid laxation .
	manualset3
219740	8	420424	7	NULL	NULL	0	NULL	effort 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Background : Opioid-induced constipation can cause great discomfort to patients who use opioids for prolonged periods and on occasion decline pain-relief in an effort to help aid laxation .
	manualset3
219741	9	420424	7	NULL	NULL	0	NULL	laxation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Background : Opioid-induced constipation can cause great discomfort to patients who use opioids for prolonged periods and on occasion decline pain-relief in an effort to help aid laxation .
	manualset3
219742	10	420424	7	NULL	NULL	0	NULL	prolonged periods	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Background : Opioid-induced constipation can cause great discomfort to patients who use opioids for prolonged periods and on occasion decline pain-relief in an effort to help aid laxation .
	manualset3
219743	1	420425	7	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of receptor mRNA was 65 - to 300-fold less than that of beta-actin mRNA .
	manualset3
219788	2	420425	7	NULL	NULL	0	NULL	receptor mRNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of receptor mRNA was 65 - to 300-fold less than that of beta-actin mRNA .
	manualset3
219795	3	420425	7	NULL	NULL	0	NULL	65 - to 300-fold 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of receptor mRNA was 65 - to 300-fold less than that of beta-actin mRNA .
	manualset3
219796	4	420425	7	NULL	NULL	0	NULL	beta-actin mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of receptor mRNA was 65 - to 300-fold less than that of beta-actin mRNA .
	manualset3
219798	1	420426	7	NULL	NULL	0	NULL	rates of referral	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The rates of referral among practitioners varied from 0 to 28.1 per 100 patients visits .
	manualset3
219801	2	420426	7	NULL	NULL	0	NULL	practitioners	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The rates of referral among practitioners varied from 0 to 28.1 per 100 patients visits .
	manualset3
219805	3	420426	7	NULL	NULL	0	NULL	0 to 28.1 per 100 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The rates of referral among practitioners varied from 0 to 28.1 per 100 patients visits .
	manualset3
219808	4	420426	7	NULL	NULL	0	NULL	visits	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The rates of referral among practitioners varied from 0 to 28.1 per 100 patients visits .
	manualset3
219812	1	420427	7	NULL	NULL	0	NULL	 paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , this paper discusses data supporting a notion that the transcription factor AP-2 family is involved in the regulation of the monoaminergic systems both pre - and postnatally , and , therefore , might be involved in the pathophysiology of neuropsychiatric disorders .
	manualset3
219816	2	420427	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , this paper discusses data supporting a notion that the transcription factor AP-2 family is involved in the regulation of the monoaminergic systems both pre - and postnatally , and , therefore , might be involved in the pathophysiology of neuropsychiatric disorders .
	manualset3
219818	3	420427	7	NULL	NULL	0	NULL	notion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , this paper discusses data supporting a notion that the transcription factor AP-2 family is involved in the regulation of the monoaminergic systems both pre - and postnatally , and , therefore , might be involved in the pathophysiology of neuropsychiatric disorders .
	manualset3
219820	4	420427	7	NULL	NULL	0	NULL	 transcription factor AP-2 family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , this paper discusses data supporting a notion that the transcription factor AP-2 family is involved in the regulation of the monoaminergic systems both pre - and postnatally , and , therefore , might be involved in the pathophysiology of neuropsychiatric disorders .
	manualset3
219821	5	420427	7	NULL	NULL	0	NULL	regulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , this paper discusses data supporting a notion that the transcription factor AP-2 family is involved in the regulation of the monoaminergic systems both pre - and postnatally , and , therefore , might be involved in the pathophysiology of neuropsychiatric disorders .
	manualset3
219822	6	420427	7	NULL	NULL	0	NULL	monoaminergic systems	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , this paper discusses data supporting a notion that the transcription factor AP-2 family is involved in the regulation of the monoaminergic systems both pre - and postnatally , and , therefore , might be involved in the pathophysiology of neuropsychiatric disorders .
	manualset3
219823	7	420427	7	NULL	NULL	0	NULL	pathophysiology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , this paper discusses data supporting a notion that the transcription factor AP-2 family is involved in the regulation of the monoaminergic systems both pre - and postnatally , and , therefore , might be involved in the pathophysiology of neuropsychiatric disorders .
	manualset3
219824	8	420427	7	NULL	NULL	0	NULL	neuropsychiatric disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether , this paper discusses data supporting a notion that the transcription factor AP-2 family is involved in the regulation of the monoaminergic systems both pre - and postnatally , and , therefore , might be involved in the pathophysiology of neuropsychiatric disorders .
	manualset3
219825	1	420428	7	NULL	NULL	0	NULL	Six horses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Six horses had primary closure of the incision , whereas six horses had a plastic mesh sutured to the ventral abdominal wall leaving the abdomen open for ventral drainage .
	manualset3
219826	2	420428	7	NULL	NULL	0	NULL	primary closure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Six horses had primary closure of the incision , whereas six horses had a plastic mesh sutured to the ventral abdominal wall leaving the abdomen open for ventral drainage .
	manualset3
219827	3	420428	7	NULL	NULL	0	NULL	incision	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Six horses had primary closure of the incision , whereas six horses had a plastic mesh sutured to the ventral abdominal wall leaving the abdomen open for ventral drainage .
	manualset3
219828	4	420428	7	NULL	NULL	0	NULL	six horses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Six horses had primary closure of the incision , whereas six horses had a plastic mesh sutured to the ventral abdominal wall leaving the abdomen open for ventral drainage .
	manualset3
219829	5	420428	7	NULL	NULL	0	NULL	plastic mesh	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Six horses had primary closure of the incision , whereas six horses had a plastic mesh sutured to the ventral abdominal wall leaving the abdomen open for ventral drainage .
	manualset3
219830	6	420428	7	NULL	NULL	0	NULL	ventral abdominal wall	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Six horses had primary closure of the incision , whereas six horses had a plastic mesh sutured to the ventral abdominal wall leaving the abdomen open for ventral drainage .
	manualset3
219831	7	420428	7	NULL	NULL	0	NULL	abdomen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Six horses had primary closure of the incision , whereas six horses had a plastic mesh sutured to the ventral abdominal wall leaving the abdomen open for ventral drainage .
	manualset3
219832	8	420428	7	NULL	NULL	0	NULL	 ventral drainage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Six horses had primary closure of the incision , whereas six horses had a plastic mesh sutured to the ventral abdominal wall leaving the abdomen open for ventral drainage .
	manualset3
219833	1	420429	7	NULL	NULL	0	NULL	Bis ( azido-N ) ( 1 , 10-phenanthroline-N , N ' ) palladium ( II )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Bis ( azido-N ) ( 1 , 10-phenanthroline-N , N ' ) palladium ( II ) .
	manualset3
219834	1	420430	7	NULL	NULL	0	NULL	Pathogenesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Pathogenesis of Osler-Rendu disease ) .
	manualset3
219835	2	420430	7	NULL	NULL	0	NULL	Osler-Rendu disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Pathogenesis of Osler-Rendu disease ) .
	manualset3
219836	1	420431	7	NULL	NULL	0	NULL	Postpartum atony	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Postpartum atony remains the most common cause life-threatening hemorrhage in obstetrics .
	manualset3
219842	2	420431	7	NULL	NULL	0	NULL	common cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Postpartum atony remains the most common cause life-threatening hemorrhage in obstetrics .
	manualset3
219843	3	420431	7	NULL	NULL	NULL	NULL	life-threatening hemorrhage	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Postpartum atony remains the most common cause life-threatening hemorrhage in obstetrics .
	manualset3
219844	4	420431	7	NULL	NULL	0	NULL	obstetrics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Postpartum atony remains the most common cause life-threatening hemorrhage in obstetrics .
	manualset3
219845	1	420432	7	NULL	NULL	0	NULL	Two cDNAs 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cDNAs complementary to the GGT mRNA have been isolated from a human placental library constructed in phage lambda gt11 .
	manualset3
219846	2	420432	7	NULL	NULL	0	NULL	GGT mRNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cDNAs complementary to the GGT mRNA have been isolated from a human placental library constructed in phage lambda gt11 .
	manualset3
219847	3	420432	7	NULL	NULL	0	NULL	human placental library 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cDNAs complementary to the GGT mRNA have been isolated from a human placental library constructed in phage lambda gt11 .
	manualset3
219848	4	420432	7	NULL	NULL	0	NULL	phage lambda gt11 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cDNAs complementary to the GGT mRNA have been isolated from a human placental library constructed in phage lambda gt11 .
	manualset3
219849	1	420433	7	NULL	NULL	0	NULL	Value	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Value of a CD-ROM and a play station ) .
	manualset3
219850	2	420433	7	NULL	NULL	0	NULL	CD-ROM	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Value of a CD-ROM and a play station ) .
	manualset3
219851	3	420433	7	NULL	NULL	0	NULL	play station 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Value of a CD-ROM and a play station ) .
	manualset3
219852	1	420434	7	NULL	NULL	0	NULL	observations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether these observations lead us to conclude that cerebellar cells in an organotypic context may be less susceptible to damage by A , raising the question whether isolated CGCs are a reliable assay in drug discovery studies of AD .
	manualset3
219853	2	420434	7	NULL	NULL	0	NULL	cerebellar cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether these observations lead us to conclude that cerebellar cells in an organotypic context may be less susceptible to damage by A , raising the question whether isolated CGCs are a reliable assay in drug discovery studies of AD .
	manualset3
219854	3	420434	7	NULL	NULL	0	NULL	organotypic context	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether these observations lead us to conclude that cerebellar cells in an organotypic context may be less susceptible to damage by A , raising the question whether isolated CGCs are a reliable assay in drug discovery studies of AD .
	manualset3
219855	4	420434	7	NULL	NULL	0	NULL	 A	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether these observations lead us to conclude that cerebellar cells in an organotypic context may be less susceptible to damage by A , raising the question whether isolated CGCs are a reliable assay in drug discovery studies of AD .
	manualset3
219856	5	420434	7	NULL	NULL	0	NULL	question 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether these observations lead us to conclude that cerebellar cells in an organotypic context may be less susceptible to damage by A , raising the question whether isolated CGCs are a reliable assay in drug discovery studies of AD .
	manualset3
219857	6	420434	7	NULL	NULL	0	NULL	isolated CGCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether these observations lead us to conclude that cerebellar cells in an organotypic context may be less susceptible to damage by A , raising the question whether isolated CGCs are a reliable assay in drug discovery studies of AD .
	manualset3
219858	7	420434	7	NULL	NULL	0	NULL	reliable assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether these observations lead us to conclude that cerebellar cells in an organotypic context may be less susceptible to damage by A , raising the question whether isolated CGCs are a reliable assay in drug discovery studies of AD .
	manualset3
219859	8	420434	7	NULL	NULL	0	NULL	drug discovery studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether these observations lead us to conclude that cerebellar cells in an organotypic context may be less susceptible to damage by A , raising the question whether isolated CGCs are a reliable assay in drug discovery studies of AD .
	manualset3
219860	9	420434	7	NULL	NULL	0	NULL	AD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether these observations lead us to conclude that cerebellar cells in an organotypic context may be less susceptible to damage by A , raising the question whether isolated CGCs are a reliable assay in drug discovery studies of AD .
	manualset3
219861	1	420435	7	NULL	NULL	0	NULL	Microencapsulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Microencapsulation of avocado oil by spray drying using whey protein and maltodextrin .
	manualset3
219862	2	420435	7	NULL	NULL	0	NULL	avocado oil 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Microencapsulation of avocado oil by spray drying using whey protein and maltodextrin .
	manualset3
219863	3	420435	7	NULL	NULL	0	NULL	spray drying 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Microencapsulation of avocado oil by spray drying using whey protein and maltodextrin .
	manualset3
219864	4	420435	7	NULL	NULL	0	NULL	whey protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Microencapsulation of avocado oil by spray drying using whey protein and maltodextrin .
	manualset3
219865	5	420435	7	NULL	NULL	0	NULL	maltodextrin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Microencapsulation of avocado oil by spray drying using whey protein and maltodextrin .
	manualset3
219866	1	420436	7	NULL	NULL	0	NULL	FE	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	FE also inhibited gastric lesion formation in a dose-dependent manner .
	manualset3
219867	2	420436	7	NULL	NULL	0	NULL	gastric lesion formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	FE also inhibited gastric lesion formation in a dose-dependent manner .
	manualset3
219868	3	420436	7	NULL	NULL	0	NULL	dose-dependent manner	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	FE also inhibited gastric lesion formation in a dose-dependent manner .
	manualset3
219869	1	420437	7	NULL	NULL	0	NULL	Human blood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Human blood : air , human and rat tissue ( fat , brain , liver , muscle , and kidney ) : air partition coefficients of a diverse set of organic compounds were correlated and predicted using structural descriptors by employing CODESSA-PRO and ISIDA programs .
	manualset3
219870	2	420437	7	NULL	NULL	0	NULL	air	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Human blood : air , human and rat tissue ( fat , brain , liver , muscle , and kidney ) : air partition coefficients of a diverse set of organic compounds were correlated and predicted using structural descriptors by employing CODESSA-PRO and ISIDA programs .
	manualset3
219871	3	420437	7	NULL	NULL	NULL	NULL	human tissue	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human blood : air , human and rat tissue ( fat , brain , liver , muscle , and kidney ) : air partition coefficients of a diverse set of organic compounds were correlated and predicted using structural descriptors by employing CODESSA-PRO and ISIDA programs .
	manualset3
219872	4	420437	7	NULL	NULL	NULL	NULL	rat tissue	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human blood : air , human and rat tissue ( fat , brain , liver , muscle , and kidney ) : air partition coefficients of a diverse set of organic compounds were correlated and predicted using structural descriptors by employing CODESSA-PRO and ISIDA programs .
	manualset3
219873	5	420437	7	NULL	NULL	NULL	NULL	fat	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Human blood : air , human and rat tissue ( fat , brain , liver , muscle , and kidney ) : air partition coefficients of a diverse set of organic compounds were correlated and predicted using structural descriptors by employing CODESSA-PRO and ISIDA programs .
	manualset3
219874	6	420437	7	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Human blood : air , human and rat tissue ( fat , brain , liver , muscle , and kidney ) : air partition coefficients of a diverse set of organic compounds were correlated and predicted using structural descriptors by employing CODESSA-PRO and ISIDA programs .
	manualset3
219875	7	420437	7	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Human blood : air , human and rat tissue ( fat , brain , liver , muscle , and kidney ) : air partition coefficients of a diverse set of organic compounds were correlated and predicted using structural descriptors by employing CODESSA-PRO and ISIDA programs .
	manualset3
219876	8	420437	7	NULL	NULL	0	NULL	muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Human blood : air , human and rat tissue ( fat , brain , liver , muscle , and kidney ) : air partition coefficients of a diverse set of organic compounds were correlated and predicted using structural descriptors by employing CODESSA-PRO and ISIDA programs .
	manualset3
219877	9	420437	7	NULL	NULL	0	NULL	kidney	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Human blood : air , human and rat tissue ( fat , brain , liver , muscle , and kidney ) : air partition coefficients of a diverse set of organic compounds were correlated and predicted using structural descriptors by employing CODESSA-PRO and ISIDA programs .
	manualset3
219878	10	420437	7	NULL	NULL	0	NULL	air partition coefficients	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Human blood : air , human and rat tissue ( fat , brain , liver , muscle , and kidney ) : air partition coefficients of a diverse set of organic compounds were correlated and predicted using structural descriptors by employing CODESSA-PRO and ISIDA programs .
	manualset3
219879	11	420437	7	NULL	NULL	0	NULL	 diverse set	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Human blood : air , human and rat tissue ( fat , brain , liver , muscle , and kidney ) : air partition coefficients of a diverse set of organic compounds were correlated and predicted using structural descriptors by employing CODESSA-PRO and ISIDA programs .
	manualset3
219880	12	420437	7	NULL	NULL	0	NULL	organic compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Human blood : air , human and rat tissue ( fat , brain , liver , muscle , and kidney ) : air partition coefficients of a diverse set of organic compounds were correlated and predicted using structural descriptors by employing CODESSA-PRO and ISIDA programs .
	manualset3
219881	13	420437	7	NULL	NULL	0	NULL	structural descriptors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Human blood : air , human and rat tissue ( fat , brain , liver , muscle , and kidney ) : air partition coefficients of a diverse set of organic compounds were correlated and predicted using structural descriptors by employing CODESSA-PRO and ISIDA programs .
	manualset3
219882	14	420437	7	NULL	NULL	0	NULL	CODESSA-PRO programs	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Human blood : air , human and rat tissue ( fat , brain , liver , muscle , and kidney ) : air partition coefficients of a diverse set of organic compounds were correlated and predicted using structural descriptors by employing CODESSA-PRO and ISIDA programs .
	manualset3
219883	15	420437	7	NULL	NULL	0	NULL	ISIDA programs	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Human blood : air , human and rat tissue ( fat , brain , liver , muscle , and kidney ) : air partition coefficients of a diverse set of organic compounds were correlated and predicted using structural descriptors by employing CODESSA-PRO and ISIDA programs .
	manualset3
219884	1	420438	7	NULL	NULL	0	NULL	Calculation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Calculation of the inherent flaw size ( ao ) from these properties produced conflicting dependencies on the state of cure .
	manualset3
219885	2	420438	7	NULL	NULL	0	NULL	inherent flaw size ( ao )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Calculation of the inherent flaw size ( ao ) from these properties produced conflicting dependencies on the state of cure .
	manualset3
219886	3	420438	7	NULL	NULL	NULL	NULL	properties	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Calculation of the inherent flaw size ( ao ) from these properties produced conflicting dependencies on the state of cure .
	manualset3
219887	4	420438	7	NULL	NULL	NULL	NULL	 conflicting dependencies	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Calculation of the inherent flaw size ( ao ) from these properties produced conflicting dependencies on the state of cure .
	manualset3
219888	5	420438	7	NULL	NULL	0	NULL	state of cure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Calculation of the inherent flaw size ( ao ) from these properties produced conflicting dependencies on the state of cure .
	manualset3
219889	1	420439	7	NULL	NULL	0	NULL	case	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of a 34-year-old woman with both pyostomatitis vegetans and primary sclerosing cholangitis is reported and the literature reviewed .
	manualset3
219890	2	420439	7	NULL	NULL	0	NULL	34-year-old woman 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of a 34-year-old woman with both pyostomatitis vegetans and primary sclerosing cholangitis is reported and the literature reviewed .
	manualset3
219891	3	420439	7	NULL	NULL	0	NULL	pyostomatitis vegetans 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of a 34-year-old woman with both pyostomatitis vegetans and primary sclerosing cholangitis is reported and the literature reviewed .
	manualset3
219892	4	420439	7	NULL	NULL	0	NULL	primary sclerosing cholangitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of a 34-year-old woman with both pyostomatitis vegetans and primary sclerosing cholangitis is reported and the literature reviewed .
	manualset3
219893	5	420439	7	NULL	NULL	0	NULL	literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The case of a 34-year-old woman with both pyostomatitis vegetans and primary sclerosing cholangitis is reported and the literature reviewed .
	manualset3
219894	1	420440	7	NULL	NULL	0	NULL	force	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We compute both the force and the torque transmitted to the cylinder by the surrounding liquid crystal and we find that the diagrams of both as functions of h fail to be monotonic along the escape texture .
	manualset3
219895	2	420440	7	NULL	NULL	0	NULL	torque	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We compute both the force and the torque transmitted to the cylinder by the surrounding liquid crystal and we find that the diagrams of both as functions of h fail to be monotonic along the escape texture .
	manualset3
219896	3	420440	7	NULL	NULL	0	NULL	cylinder	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	We compute both the force and the torque transmitted to the cylinder by the surrounding liquid crystal and we find that the diagrams of both as functions of h fail to be monotonic along the escape texture .
	manualset3
219897	4	420440	7	NULL	NULL	0	NULL	liquid crystal	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We compute both the force and the torque transmitted to the cylinder by the surrounding liquid crystal and we find that the diagrams of both as functions of h fail to be monotonic along the escape texture .
	manualset3
219898	5	420440	7	NULL	NULL	0	NULL	diagrams	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We compute both the force and the torque transmitted to the cylinder by the surrounding liquid crystal and we find that the diagrams of both as functions of h fail to be monotonic along the escape texture .
	manualset3
219899	6	420440	7	NULL	NULL	0	NULL	functions of h	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We compute both the force and the torque transmitted to the cylinder by the surrounding liquid crystal and we find that the diagrams of both as functions of h fail to be monotonic along the escape texture .
	manualset3
219900	7	420440	7	NULL	NULL	0	NULL	monotonic 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We compute both the force and the torque transmitted to the cylinder by the surrounding liquid crystal and we find that the diagrams of both as functions of h fail to be monotonic along the escape texture .
	manualset3
219901	8	420440	7	NULL	NULL	0	NULL	escape texture	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We compute both the force and the torque transmitted to the cylinder by the surrounding liquid crystal and we find that the diagrams of both as functions of h fail to be monotonic along the escape texture .
	manualset3
219902	1	420441	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether these results have led to the hypothesis of two major pathophysiological mechanisms in Alzheimer 's disease : on one hand compensatory mechanisms in regions where atrophy exceeds metabolic alterations , on the other disconnection between medial temporal lobe and posterior cingulate cortex through the cingulum bundle , accounting for higher metabolic than structural alterations in the posterior cingulate cortex .
	manualset3
219903	2	420441	7	NULL	NULL	0	NULL	 hypothesis 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether these results have led to the hypothesis of two major pathophysiological mechanisms in Alzheimer 's disease : on one hand compensatory mechanisms in regions where atrophy exceeds metabolic alterations , on the other disconnection between medial temporal lobe and posterior cingulate cortex through the cingulum bundle , accounting for higher metabolic than structural alterations in the posterior cingulate cortex .
	manualset3
219904	3	420441	7	NULL	NULL	0	NULL	two major pathophysiological mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether these results have led to the hypothesis of two major pathophysiological mechanisms in Alzheimer 's disease : on one hand compensatory mechanisms in regions where atrophy exceeds metabolic alterations , on the other disconnection between medial temporal lobe and posterior cingulate cortex through the cingulum bundle , accounting for higher metabolic than structural alterations in the posterior cingulate cortex .
	manualset3
219905	4	420441	7	NULL	NULL	0	NULL	Alzheimer 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether these results have led to the hypothesis of two major pathophysiological mechanisms in Alzheimer 's disease : on one hand compensatory mechanisms in regions where atrophy exceeds metabolic alterations , on the other disconnection between medial temporal lobe and posterior cingulate cortex through the cingulum bundle , accounting for higher metabolic than structural alterations in the posterior cingulate cortex .
	manualset3
219906	5	420441	7	NULL	NULL	0	NULL	one hand	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether these results have led to the hypothesis of two major pathophysiological mechanisms in Alzheimer 's disease : on one hand compensatory mechanisms in regions where atrophy exceeds metabolic alterations , on the other disconnection between medial temporal lobe and posterior cingulate cortex through the cingulum bundle , accounting for higher metabolic than structural alterations in the posterior cingulate cortex .
	manualset3
219907	6	420441	7	NULL	NULL	0	NULL	compensatory mechanisms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether these results have led to the hypothesis of two major pathophysiological mechanisms in Alzheimer 's disease : on one hand compensatory mechanisms in regions where atrophy exceeds metabolic alterations , on the other disconnection between medial temporal lobe and posterior cingulate cortex through the cingulum bundle , accounting for higher metabolic than structural alterations in the posterior cingulate cortex .
	manualset3
219908	7	420441	7	NULL	NULL	0	NULL	regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether these results have led to the hypothesis of two major pathophysiological mechanisms in Alzheimer 's disease : on one hand compensatory mechanisms in regions where atrophy exceeds metabolic alterations , on the other disconnection between medial temporal lobe and posterior cingulate cortex through the cingulum bundle , accounting for higher metabolic than structural alterations in the posterior cingulate cortex .
	manualset3
219909	8	420441	7	NULL	NULL	0	NULL	atrophy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether these results have led to the hypothesis of two major pathophysiological mechanisms in Alzheimer 's disease : on one hand compensatory mechanisms in regions where atrophy exceeds metabolic alterations , on the other disconnection between medial temporal lobe and posterior cingulate cortex through the cingulum bundle , accounting for higher metabolic than structural alterations in the posterior cingulate cortex .
	manualset3
219910	9	420441	7	NULL	NULL	0	NULL	metabolic alterations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether these results have led to the hypothesis of two major pathophysiological mechanisms in Alzheimer 's disease : on one hand compensatory mechanisms in regions where atrophy exceeds metabolic alterations , on the other disconnection between medial temporal lobe and posterior cingulate cortex through the cingulum bundle , accounting for higher metabolic than structural alterations in the posterior cingulate cortex .
	manualset3
219911	10	420441	7	NULL	NULL	NULL	NULL	disconnection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Altogether these results have led to the hypothesis of two major pathophysiological mechanisms in Alzheimer 's disease : on one hand compensatory mechanisms in regions where atrophy exceeds metabolic alterations , on the other disconnection between medial temporal lobe and posterior cingulate cortex through the cingulum bundle , accounting for higher metabolic than structural alterations in the posterior cingulate cortex .
	manualset3
219912	11	420441	7	NULL	NULL	0	NULL	medial temporal lobe	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether these results have led to the hypothesis of two major pathophysiological mechanisms in Alzheimer 's disease : on one hand compensatory mechanisms in regions where atrophy exceeds metabolic alterations , on the other disconnection between medial temporal lobe and posterior cingulate cortex through the cingulum bundle , accounting for higher metabolic than structural alterations in the posterior cingulate cortex .
	manualset3
219913	12	420441	7	NULL	NULL	NULL	NULL	posterior cingulate cortex 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Altogether these results have led to the hypothesis of two major pathophysiological mechanisms in Alzheimer 's disease : on one hand compensatory mechanisms in regions where atrophy exceeds metabolic alterations , on the other disconnection between medial temporal lobe and posterior cingulate cortex through the cingulum bundle , accounting for higher metabolic than structural alterations in the posterior cingulate cortex .
	manualset3
219914	13	420441	7	NULL	NULL	NULL	NULL	cingulum bundle	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Altogether these results have led to the hypothesis of two major pathophysiological mechanisms in Alzheimer 's disease : on one hand compensatory mechanisms in regions where atrophy exceeds metabolic alterations , on the other disconnection between medial temporal lobe and posterior cingulate cortex through the cingulum bundle , accounting for higher metabolic than structural alterations in the posterior cingulate cortex .
	manualset3
219915	15	420441	7	NULL	NULL	NULL	NULL	 posterior cingulate cortex	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Altogether these results have led to the hypothesis of two major pathophysiological mechanisms in Alzheimer 's disease : on one hand compensatory mechanisms in regions where atrophy exceeds metabolic alterations , on the other disconnection between medial temporal lobe and posterior cingulate cortex through the cingulum bundle , accounting for higher metabolic than structural alterations in the posterior cingulate cortex .
	manualset3
219916	14	420441	7	NULL	NULL	0	NULL	structural alterations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Altogether these results have led to the hypothesis of two major pathophysiological mechanisms in Alzheimer 's disease : on one hand compensatory mechanisms in regions where atrophy exceeds metabolic alterations , on the other disconnection between medial temporal lobe and posterior cingulate cortex through the cingulum bundle , accounting for higher metabolic than structural alterations in the posterior cingulate cortex .
	manualset3
219917	1	420442	7	NULL	NULL	0	NULL	lack 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The lack of accumulation of free 18 : 3 after elicitation suggests a tight physical association between GLA1 and LOX3 in N. attenuata leaves .
	manualset3
219918	2	420442	7	NULL	NULL	0	NULL	accumulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The lack of accumulation of free 18 : 3 after elicitation suggests a tight physical association between GLA1 and LOX3 in N. attenuata leaves .
	manualset3
219919	3	420442	7	NULL	NULL	0	NULL	free 18 : 3 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The lack of accumulation of free 18 : 3 after elicitation suggests a tight physical association between GLA1 and LOX3 in N. attenuata leaves .
	manualset3
219920	4	420442	7	NULL	NULL	0	NULL	elicitation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The lack of accumulation of free 18 : 3 after elicitation suggests a tight physical association between GLA1 and LOX3 in N. attenuata leaves .
	manualset3
219921	5	420442	7	NULL	NULL	0	NULL	 tight physical association	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The lack of accumulation of free 18 : 3 after elicitation suggests a tight physical association between GLA1 and LOX3 in N. attenuata leaves .
	manualset3
219922	6	420442	7	NULL	NULL	0	NULL	GLA1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The lack of accumulation of free 18 : 3 after elicitation suggests a tight physical association between GLA1 and LOX3 in N. attenuata leaves .
	manualset3
219923	7	420442	7	NULL	NULL	0	NULL	LOX3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The lack of accumulation of free 18 : 3 after elicitation suggests a tight physical association between GLA1 and LOX3 in N. attenuata leaves .
	manualset3
219924	8	420442	7	NULL	NULL	0	NULL	N. attenuata leaves	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The lack of accumulation of free 18 : 3 after elicitation suggests a tight physical association between GLA1 and LOX3 in N. attenuata leaves .
	manualset3
219925	1	420443	7	NULL	NULL	0	NULL	 paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper reviews both the data available in the literature and the authors ' own results of long-term experimental and clinical investigations of the involvement of hepatic monooxygenases ( HMO ) in the biological activity of antitumor drugs .
	manualset3
219926	2	420443	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper reviews both the data available in the literature and the authors ' own results of long-term experimental and clinical investigations of the involvement of hepatic monooxygenases ( HMO ) in the biological activity of antitumor drugs .
	manualset3
219927	3	420443	7	NULL	NULL	0	NULL	literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper reviews both the data available in the literature and the authors ' own results of long-term experimental and clinical investigations of the involvement of hepatic monooxygenases ( HMO ) in the biological activity of antitumor drugs .
	manualset3
219928	4	420443	7	NULL	NULL	0	NULL	authors ' own results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper reviews both the data available in the literature and the authors ' own results of long-term experimental and clinical investigations of the involvement of hepatic monooxygenases ( HMO ) in the biological activity of antitumor drugs .
	manualset3
219929	5	420443	7	NULL	NULL	0	NULL	long-term experimental investigations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper reviews both the data available in the literature and the authors ' own results of long-term experimental and clinical investigations of the involvement of hepatic monooxygenases ( HMO ) in the biological activity of antitumor drugs .
	manualset3
219930	6	420443	7	NULL	NULL	0	NULL	clinical investigations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper reviews both the data available in the literature and the authors ' own results of long-term experimental and clinical investigations of the involvement of hepatic monooxygenases ( HMO ) in the biological activity of antitumor drugs .
	manualset3
219931	7	420443	7	NULL	NULL	0	NULL	 involvement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper reviews both the data available in the literature and the authors ' own results of long-term experimental and clinical investigations of the involvement of hepatic monooxygenases ( HMO ) in the biological activity of antitumor drugs .
	manualset3
219932	8	420443	7	NULL	NULL	NULL	NULL	hepatic monooxygenases(HMO)	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The paper reviews both the data available in the literature and the authors ' own results of long-term experimental and clinical investigations of the involvement of hepatic monooxygenases ( HMO ) in the biological activity of antitumor drugs .
	manualset3
219933	9	420443	7	NULL	NULL	0	NULL	biological activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper reviews both the data available in the literature and the authors ' own results of long-term experimental and clinical investigations of the involvement of hepatic monooxygenases ( HMO ) in the biological activity of antitumor drugs .
	manualset3
219934	10	420443	7	NULL	NULL	0	NULL	antitumor drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The paper reviews both the data available in the literature and the authors ' own results of long-term experimental and clinical investigations of the involvement of hepatic monooxygenases ( HMO ) in the biological activity of antitumor drugs .
	manualset3
219935	1	420444	7	NULL	NULL	0	NULL	Custom abutments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Custom abutments can be more predictably formed to re-create the desired supporting preparation orientation and morphology .
	manualset3
219936	2	420444	7	NULL	NULL	0	NULL	supporting preparation orientation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Custom abutments can be more predictably formed to re-create the desired supporting preparation orientation and morphology .
	manualset3
219937	3	420444	7	NULL	NULL	0	NULL	morphology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Custom abutments can be more predictably formed to re-create the desired supporting preparation orientation and morphology .
	manualset3
219938	1	420445	7	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of these findings with those from other patients with diencephalic amnesia suggests that amnesia can result when several diencephalic structures are damaged conjointly , including the internal medullary lamina , the intralaminar nuclei , the mediodorsal nucleus , and the mammillothalamic tract .
	manualset3
219939	2	420445	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of these findings with those from other patients with diencephalic amnesia suggests that amnesia can result when several diencephalic structures are damaged conjointly , including the internal medullary lamina , the intralaminar nuclei , the mediodorsal nucleus , and the mammillothalamic tract .
	manualset3
219940	3	420445	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of these findings with those from other patients with diencephalic amnesia suggests that amnesia can result when several diencephalic structures are damaged conjointly , including the internal medullary lamina , the intralaminar nuclei , the mediodorsal nucleus , and the mammillothalamic tract .
	manualset3
219941	4	420445	7	NULL	NULL	0	NULL	diencephalic amnesia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of these findings with those from other patients with diencephalic amnesia suggests that amnesia can result when several diencephalic structures are damaged conjointly , including the internal medullary lamina , the intralaminar nuclei , the mediodorsal nucleus , and the mammillothalamic tract .
	manualset3
219942	5	420445	7	NULL	NULL	0	NULL	amnesia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of these findings with those from other patients with diencephalic amnesia suggests that amnesia can result when several diencephalic structures are damaged conjointly , including the internal medullary lamina , the intralaminar nuclei , the mediodorsal nucleus , and the mammillothalamic tract .
	manualset3
219943	6	420445	7	NULL	NULL	NULL	NULL	 diencephalic structures	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A comparison of these findings with those from other patients with diencephalic amnesia suggests that amnesia can result when several diencephalic structures are damaged conjointly , including the internal medullary lamina , the intralaminar nuclei , the mediodorsal nucleus , and the mammillothalamic tract .
	manualset3
219944	7	420445	7	NULL	NULL	0	NULL	internal medullary lamina	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of these findings with those from other patients with diencephalic amnesia suggests that amnesia can result when several diencephalic structures are damaged conjointly , including the internal medullary lamina , the intralaminar nuclei , the mediodorsal nucleus , and the mammillothalamic tract .
	manualset3
219945	8	420445	7	NULL	NULL	0	NULL	intralaminar nuclei	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of these findings with those from other patients with diencephalic amnesia suggests that amnesia can result when several diencephalic structures are damaged conjointly , including the internal medullary lamina , the intralaminar nuclei , the mediodorsal nucleus , and the mammillothalamic tract .
	manualset3
219946	9	420445	7	NULL	NULL	0	NULL	mediodorsal nucleus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of these findings with those from other patients with diencephalic amnesia suggests that amnesia can result when several diencephalic structures are damaged conjointly , including the internal medullary lamina , the intralaminar nuclei , the mediodorsal nucleus , and the mammillothalamic tract .
	manualset3
219947	10	420445	7	NULL	NULL	0	NULL	mammillothalamic tract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparison of these findings with those from other patients with diencephalic amnesia suggests that amnesia can result when several diencephalic structures are damaged conjointly , including the internal medullary lamina , the intralaminar nuclei , the mediodorsal nucleus , and the mammillothalamic tract .
	manualset3
219948	1	420446	7	NULL	NULL	0	NULL	262 , 7859-7864	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	262 , 7859-7864 ) , we demonstrated that the pro-sequence consisting of 77 amino acid residues at the amino terminus of subtilisin is essential for the production of active subtilisin .
	manualset3
219949	2	420446	7	NULL	NULL	0	NULL	pro-sequence	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	262 , 7859-7864 ) , we demonstrated that the pro-sequence consisting of 77 amino acid residues at the amino terminus of subtilisin is essential for the production of active subtilisin .
	manualset3
219950	3	420446	7	NULL	NULL	0	NULL	 77 amino acid residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	262 , 7859-7864 ) , we demonstrated that the pro-sequence consisting of 77 amino acid residues at the amino terminus of subtilisin is essential for the production of active subtilisin .
	manualset3
219951	4	420446	7	NULL	NULL	0	NULL	amino terminus	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	262 , 7859-7864 ) , we demonstrated that the pro-sequence consisting of 77 amino acid residues at the amino terminus of subtilisin is essential for the production of active subtilisin .
	manualset3
219952	5	420446	7	NULL	NULL	0	NULL	subtilisin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	262 , 7859-7864 ) , we demonstrated that the pro-sequence consisting of 77 amino acid residues at the amino terminus of subtilisin is essential for the production of active subtilisin .
	manualset3
219953	6	420446	7	NULL	NULL	0	NULL	production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	262 , 7859-7864 ) , we demonstrated that the pro-sequence consisting of 77 amino acid residues at the amino terminus of subtilisin is essential for the production of active subtilisin .
	manualset3
219954	7	420446	7	NULL	NULL	0	NULL	active subtilisin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	262 , 7859-7864 ) , we demonstrated that the pro-sequence consisting of 77 amino acid residues at the amino terminus of subtilisin is essential for the production of active subtilisin .
	manualset3
219955	1	420447	7	NULL	NULL	0	NULL	68 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We observed a 68 % , 64 % and 66 % increase in the expression of Trks A , B and C , respectively , in the ductal elements of the PDAC samples examined compared with the normal adjacent tissue .
	manualset3
219956	2	420447	7	NULL	NULL	0	NULL	64 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We observed a 68 % , 64 % and 66 % increase in the expression of Trks A , B and C , respectively , in the ductal elements of the PDAC samples examined compared with the normal adjacent tissue .
	manualset3
219957	3	420447	7	NULL	NULL	0	NULL	 66 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We observed a 68 % , 64 % and 66 % increase in the expression of Trks A , B and C , respectively , in the ductal elements of the PDAC samples examined compared with the normal adjacent tissue .
	manualset3
219958	4	420447	7	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We observed a 68 % , 64 % and 66 % increase in the expression of Trks A , B and C , respectively , in the ductal elements of the PDAC samples examined compared with the normal adjacent tissue .
	manualset3
219959	5	420447	7	NULL	NULL	0	NULL	Trks A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We observed a 68 % , 64 % and 66 % increase in the expression of Trks A , B and C , respectively , in the ductal elements of the PDAC samples examined compared with the normal adjacent tissue .
	manualset3
219960	6	420447	7	NULL	NULL	0	NULL	Trks B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We observed a 68 % , 64 % and 66 % increase in the expression of Trks A , B and C , respectively , in the ductal elements of the PDAC samples examined compared with the normal adjacent tissue .
	manualset3
219961	7	420447	7	NULL	NULL	0	NULL	Trks C	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We observed a 68 % , 64 % and 66 % increase in the expression of Trks A , B and C , respectively , in the ductal elements of the PDAC samples examined compared with the normal adjacent tissue .
	manualset3
219962	8	420447	7	NULL	NULL	0	NULL	ductal elements	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We observed a 68 % , 64 % and 66 % increase in the expression of Trks A , B and C , respectively , in the ductal elements of the PDAC samples examined compared with the normal adjacent tissue .
	manualset3
219963	9	420447	7	NULL	NULL	0	NULL	PDAC samples 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We observed a 68 % , 64 % and 66 % increase in the expression of Trks A , B and C , respectively , in the ductal elements of the PDAC samples examined compared with the normal adjacent tissue .
	manualset3
219964	10	420447	7	NULL	NULL	0	NULL	normal adjacent tissue 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	We observed a 68 % , 64 % and 66 % increase in the expression of Trks A , B and C , respectively , in the ductal elements of the PDAC samples examined compared with the normal adjacent tissue .
	manualset3
219965	1	420448	7	NULL	NULL	0	NULL	 5 cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 5 cases of moderate shrinkage , the reduction occurred progressively for 1 year .
	manualset3
219966	2	420448	7	NULL	NULL	0	NULL	moderate shrinkage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 5 cases of moderate shrinkage , the reduction occurred progressively for 1 year .
	manualset3
219967	3	420448	7	NULL	NULL	0	NULL	 reduction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 5 cases of moderate shrinkage , the reduction occurred progressively for 1 year .
	manualset3
219968	4	420448	7	NULL	NULL	0	NULL	1 year	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the 5 cases of moderate shrinkage , the reduction occurred progressively for 1 year .
	manualset3
219969	1	420449	7	NULL	NULL	0	NULL	Peptides 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptides corresponding to the C-terminal heptad repeat of HIV-1 gp41 ( C-peptides ) are potent inhibitors of HIV-1 entry into cells .
	manualset3
219970	2	420449	7	NULL	NULL	0	NULL	C-terminal heptad repeat	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptides corresponding to the C-terminal heptad repeat of HIV-1 gp41 ( C-peptides ) are potent inhibitors of HIV-1 entry into cells .
	manualset3
219971	3	420449	7	NULL	NULL	0	NULL	HIV-1 gp41 ( C-peptides ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptides corresponding to the C-terminal heptad repeat of HIV-1 gp41 ( C-peptides ) are potent inhibitors of HIV-1 entry into cells .
	manualset3
219972	4	420449	7	NULL	NULL	0	NULL	potent inhibitors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptides corresponding to the C-terminal heptad repeat of HIV-1 gp41 ( C-peptides ) are potent inhibitors of HIV-1 entry into cells .
	manualset3
219973	5	420449	7	NULL	NULL	0	NULL	HIV-1 entry 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptides corresponding to the C-terminal heptad repeat of HIV-1 gp41 ( C-peptides ) are potent inhibitors of HIV-1 entry into cells .
	manualset3
219974	6	420449	7	NULL	NULL	0	NULL	 cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Peptides corresponding to the C-terminal heptad repeat of HIV-1 gp41 ( C-peptides ) are potent inhibitors of HIV-1 entry into cells .
	manualset3
219975	1	420450	7	NULL	NULL	0	NULL	HPLC methodology	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	HPLC and TLC methodology for determination or purity evaluation of 4-methoxy-2 - ( 3 ( 4-phenyl-1-piperazinyl ) ) propyl-2 , 3 - dihydro-6-methyl-1 , 3 - dioxo-1H-pyrrolo ( 3 , 4-c ) pyridine .
	manualset3
219976	2	420450	7	NULL	NULL	0	NULL	TLC methodology	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	HPLC and TLC methodology for determination or purity evaluation of 4-methoxy-2 - ( 3 ( 4-phenyl-1-piperazinyl ) ) propyl-2 , 3 - dihydro-6-methyl-1 , 3 - dioxo-1H-pyrrolo ( 3 , 4-c ) pyridine .
	manualset3
219977	3	420450	7	NULL	NULL	0	NULL	determination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	HPLC and TLC methodology for determination or purity evaluation of 4-methoxy-2 - ( 3 ( 4-phenyl-1-piperazinyl ) ) propyl-2 , 3 - dihydro-6-methyl-1 , 3 - dioxo-1H-pyrrolo ( 3 , 4-c ) pyridine .
	manualset3
219978	4	420450	7	NULL	NULL	0	NULL	purity evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	HPLC and TLC methodology for determination or purity evaluation of 4-methoxy-2 - ( 3 ( 4-phenyl-1-piperazinyl ) ) propyl-2 , 3 - dihydro-6-methyl-1 , 3 - dioxo-1H-pyrrolo ( 3 , 4-c ) pyridine .
	manualset3
219979	5	420450	7	NULL	NULL	0	NULL	4-methoxy-2 - ( 3 ( 4-phenyl-1-piperazinyl ) ) propyl-2 , 3 - dihydro-6-methyl-1 , 3 - dioxo-1H-pyrrolo ( 3 , 4-c ) pyridine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	HPLC and TLC methodology for determination or purity evaluation of 4-methoxy-2 - ( 3 ( 4-phenyl-1-piperazinyl ) ) propyl-2 , 3 - dihydro-6-methyl-1 , 3 - dioxo-1H-pyrrolo ( 3 , 4-c ) pyridine .
	manualset3
219980	1	420451	7	NULL	NULL	0	NULL	early orthodontic treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	So it is very important to start an early orthodontic treatment to avoid the periodontal consequences of malocclusion before it has become irreversible .
	manualset3
219981	2	420451	7	NULL	NULL	0	NULL	periodontal consequences	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	So it is very important to start an early orthodontic treatment to avoid the periodontal consequences of malocclusion before it has become irreversible .
	manualset3
219982	3	420451	7	NULL	NULL	0	NULL	 malocclusion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	So it is very important to start an early orthodontic treatment to avoid the periodontal consequences of malocclusion before it has become irreversible .
	manualset3
219983	4	420451	7	NULL	NULL	0	NULL	irreversible	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	So it is very important to start an early orthodontic treatment to avoid the periodontal consequences of malocclusion before it has become irreversible .
	manualset3
219984	1	420452	7	NULL	NULL	0	NULL	( 3H ) A-69024	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3H ) A-69024 : a non-benzazepine ligand for in vitro and in vivo studies of dopamine D1 receptors .
	manualset3
219985	2	420452	7	NULL	NULL	0	NULL	non-benzazepine ligand	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3H ) A-69024 : a non-benzazepine ligand for in vitro and in vivo studies of dopamine D1 receptors .
	manualset3
219986	3	420452	7	NULL	NULL	0	NULL	in vitro studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3H ) A-69024 : a non-benzazepine ligand for in vitro and in vivo studies of dopamine D1 receptors .
	manualset3
219987	4	420452	7	NULL	NULL	0	NULL	in vivo studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3H ) A-69024 : a non-benzazepine ligand for in vitro and in vivo studies of dopamine D1 receptors .
	manualset3
219988	5	420452	7	NULL	NULL	0	NULL	dopamine D1 receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( 3H ) A-69024 : a non-benzazepine ligand for in vitro and in vivo studies of dopamine D1 receptors .
	manualset3
219989	1	420453	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although expression by epithelial cells of some antimicrobial peptides ( e.g. , beta-defensins ) of humans and ruminants is increased in response to acute infection , AP expression is not increased during acute infection , which suggests that the expression of the latter peptide is constitutive .
	manualset3
219990	2	420453	7	NULL	NULL	0	NULL	epithelial cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Although expression by epithelial cells of some antimicrobial peptides ( e.g. , beta-defensins ) of humans and ruminants is increased in response to acute infection , AP expression is not increased during acute infection , which suggests that the expression of the latter peptide is constitutive .
	manualset3
219991	3	420453	7	NULL	NULL	0	NULL	antimicrobial peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Although expression by epithelial cells of some antimicrobial peptides ( e.g. , beta-defensins ) of humans and ruminants is increased in response to acute infection , AP expression is not increased during acute infection , which suggests that the expression of the latter peptide is constitutive .
	manualset3
219992	4	420453	7	NULL	NULL	0	NULL	 beta-defensins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although expression by epithelial cells of some antimicrobial peptides ( e.g. , beta-defensins ) of humans and ruminants is increased in response to acute infection , AP expression is not increased during acute infection , which suggests that the expression of the latter peptide is constitutive .
	manualset3
219993	5	420453	7	NULL	NULL	0	NULL	humans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although expression by epithelial cells of some antimicrobial peptides ( e.g. , beta-defensins ) of humans and ruminants is increased in response to acute infection , AP expression is not increased during acute infection , which suggests that the expression of the latter peptide is constitutive .
	manualset3
219994	6	420453	7	NULL	NULL	0	NULL	ruminants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although expression by epithelial cells of some antimicrobial peptides ( e.g. , beta-defensins ) of humans and ruminants is increased in response to acute infection , AP expression is not increased during acute infection , which suggests that the expression of the latter peptide is constitutive .
	manualset3
219995	7	420453	7	NULL	NULL	0	NULL	acute infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although expression by epithelial cells of some antimicrobial peptides ( e.g. , beta-defensins ) of humans and ruminants is increased in response to acute infection , AP expression is not increased during acute infection , which suggests that the expression of the latter peptide is constitutive .
	manualset3
219996	8	420453	7	NULL	NULL	0	NULL	AP expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although expression by epithelial cells of some antimicrobial peptides ( e.g. , beta-defensins ) of humans and ruminants is increased in response to acute infection , AP expression is not increased during acute infection , which suggests that the expression of the latter peptide is constitutive .
	manualset3
219997	9	420453	7	NULL	NULL	0	NULL	acute infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although expression by epithelial cells of some antimicrobial peptides ( e.g. , beta-defensins ) of humans and ruminants is increased in response to acute infection , AP expression is not increased during acute infection , which suggests that the expression of the latter peptide is constitutive .
	manualset3
219998	10	420453	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although expression by epithelial cells of some antimicrobial peptides ( e.g. , beta-defensins ) of humans and ruminants is increased in response to acute infection , AP expression is not increased during acute infection , which suggests that the expression of the latter peptide is constitutive .
	manualset3
219999	11	420453	7	NULL	NULL	0	NULL	peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Although expression by epithelial cells of some antimicrobial peptides ( e.g. , beta-defensins ) of humans and ruminants is increased in response to acute infection , AP expression is not increased during acute infection , which suggests that the expression of the latter peptide is constitutive .
	manualset3
220000	1	420454	7	NULL	NULL	0	NULL	Epidemiological assessment 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiological assessment of liver disease in northeastern Brazil by means of a standardized liver biopsy protocol .
	manualset3
220001	2	420454	7	NULL	NULL	0	NULL	liver disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiological assessment of liver disease in northeastern Brazil by means of a standardized liver biopsy protocol .
	manualset3
220002	3	420454	7	NULL	NULL	0	NULL	northeastern Brazil 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiological assessment of liver disease in northeastern Brazil by means of a standardized liver biopsy protocol .
	manualset3
220003	4	420454	7	NULL	NULL	0	NULL	standardized liver biopsy protocol	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiological assessment of liver disease in northeastern Brazil by means of a standardized liver biopsy protocol .
	manualset3
220004	1	420455	7	NULL	NULL	0	NULL	S ( f )	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Since both S ( f ) and ( g-1 ( t ) ) 2 lacked frequency components lower than 1 / ( 2048T ) Hz , their profiles were highly reproducible .
	manualset3
220005	2	420455	7	NULL	NULL	0	NULL	( g-1 ( t ) ) 2	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Since both S ( f ) and ( g-1 ( t ) ) 2 lacked frequency components lower than 1 / ( 2048T ) Hz , their profiles were highly reproducible .
	manualset3
220006	3	420455	7	NULL	NULL	NULL	NULL	frequency components	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Since both S ( f ) and ( g-1 ( t ) ) 2 lacked frequency components lower than 1 / ( 2048T ) Hz , their profiles were highly reproducible .
	manualset3
220007	4	420455	7	NULL	NULL	0	NULL	1 / ( 2048T ) Hz	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since both S ( f ) and ( g-1 ( t ) ) 2 lacked frequency components lower than 1 / ( 2048T ) Hz , their profiles were highly reproducible .
	manualset3
220008	5	420455	7	NULL	NULL	0	NULL	profiles	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Since both S ( f ) and ( g-1 ( t ) ) 2 lacked frequency components lower than 1 / ( 2048T ) Hz , their profiles were highly reproducible .
	manualset3
220009	1	420456	7	NULL	NULL	0	NULL	Elevated proline aminopeptidase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Elevated proline aminopeptidase activity has been identified as a reliable marker enzyme for bacterial vaginosis .
	manualset3
220010	2	420456	7	NULL	NULL	0	NULL	reliable marker enzyme	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Elevated proline aminopeptidase activity has been identified as a reliable marker enzyme for bacterial vaginosis .
	manualset3
220011	3	420456	7	NULL	NULL	0	NULL	bacterial vaginosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Elevated proline aminopeptidase activity has been identified as a reliable marker enzyme for bacterial vaginosis .
	manualset3
220012	1	420457	7	NULL	NULL	0	NULL	14 bulls 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For 14 bulls the BLAD genotype was not indicated .
	manualset3
220013	2	420457	7	NULL	NULL	0	NULL	BLAD genotype	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	For 14 bulls the BLAD genotype was not indicated .
	manualset3
220014	1	420458	7	NULL	NULL	0	NULL	Endoscopic assessment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Endoscopic assessment for the presence of erosion and hemorrhage after 1 and 2 weeks of famotidine treatment showed that the 10 - and 20-mg doses were more effective in healing erosions and hemorrhages than was the 5-mg dose .
	manualset3
220015	2	420458	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Endoscopic assessment for the presence of erosion and hemorrhage after 1 and 2 weeks of famotidine treatment showed that the 10 - and 20-mg doses were more effective in healing erosions and hemorrhages than was the 5-mg dose .
	manualset3
220016	3	420458	7	NULL	NULL	0	NULL	erosion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Endoscopic assessment for the presence of erosion and hemorrhage after 1 and 2 weeks of famotidine treatment showed that the 10 - and 20-mg doses were more effective in healing erosions and hemorrhages than was the 5-mg dose .
	manualset3
220017	4	420458	7	NULL	NULL	0	NULL	hemorrhage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Endoscopic assessment for the presence of erosion and hemorrhage after 1 and 2 weeks of famotidine treatment showed that the 10 - and 20-mg doses were more effective in healing erosions and hemorrhages than was the 5-mg dose .
	manualset3
220018	5	420458	7	NULL	NULL	0	NULL	1 week	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Endoscopic assessment for the presence of erosion and hemorrhage after 1 and 2 weeks of famotidine treatment showed that the 10 - and 20-mg doses were more effective in healing erosions and hemorrhages than was the 5-mg dose .
	manualset3
220019	6	420458	7	NULL	NULL	0	NULL	2 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Endoscopic assessment for the presence of erosion and hemorrhage after 1 and 2 weeks of famotidine treatment showed that the 10 - and 20-mg doses were more effective in healing erosions and hemorrhages than was the 5-mg dose .
	manualset3
220020	7	420458	7	NULL	NULL	0	NULL	famotidine treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Endoscopic assessment for the presence of erosion and hemorrhage after 1 and 2 weeks of famotidine treatment showed that the 10 - and 20-mg doses were more effective in healing erosions and hemorrhages than was the 5-mg dose .
	manualset3
220021	8	420458	7	NULL	NULL	0	NULL	10 -mg doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Endoscopic assessment for the presence of erosion and hemorrhage after 1 and 2 weeks of famotidine treatment showed that the 10 - and 20-mg doses were more effective in healing erosions and hemorrhages than was the 5-mg dose .
	manualset3
220022	9	420458	7	NULL	NULL	0	NULL	20-mg doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Endoscopic assessment for the presence of erosion and hemorrhage after 1 and 2 weeks of famotidine treatment showed that the 10 - and 20-mg doses were more effective in healing erosions and hemorrhages than was the 5-mg dose .
	manualset3
220023	10	420458	7	NULL	NULL	0	NULL	healing erosions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Endoscopic assessment for the presence of erosion and hemorrhage after 1 and 2 weeks of famotidine treatment showed that the 10 - and 20-mg doses were more effective in healing erosions and hemorrhages than was the 5-mg dose .
	manualset3
220024	11	420458	7	NULL	NULL	0	NULL	hemorrhages	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Endoscopic assessment for the presence of erosion and hemorrhage after 1 and 2 weeks of famotidine treatment showed that the 10 - and 20-mg doses were more effective in healing erosions and hemorrhages than was the 5-mg dose .
	manualset3
220025	12	420458	7	NULL	NULL	0	NULL	 5-mg dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Endoscopic assessment for the presence of erosion and hemorrhage after 1 and 2 weeks of famotidine treatment showed that the 10 - and 20-mg doses were more effective in healing erosions and hemorrhages than was the 5-mg dose .
	manualset3
220026	1	420459	7	NULL	NULL	0	NULL	solution structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The solution structure of the complex was calculated by means of hybrid distance geometry-simulated annealing using a combination of experimental NMR restraints obtained from the previous refinement of the inhibitor-free MMP-1 ( 1 ) and recent restraints for the MMP-1 : CGS-27023A complex .
	manualset3
220027	2	420459	7	NULL	NULL	0	NULL	complex 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The solution structure of the complex was calculated by means of hybrid distance geometry-simulated annealing using a combination of experimental NMR restraints obtained from the previous refinement of the inhibitor-free MMP-1 ( 1 ) and recent restraints for the MMP-1 : CGS-27023A complex .
	manualset3
220028	3	420459	7	NULL	NULL	0	NULL	hybrid distance geometry-simulated annealing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The solution structure of the complex was calculated by means of hybrid distance geometry-simulated annealing using a combination of experimental NMR restraints obtained from the previous refinement of the inhibitor-free MMP-1 ( 1 ) and recent restraints for the MMP-1 : CGS-27023A complex .
	manualset3
220029	4	420459	7	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The solution structure of the complex was calculated by means of hybrid distance geometry-simulated annealing using a combination of experimental NMR restraints obtained from the previous refinement of the inhibitor-free MMP-1 ( 1 ) and recent restraints for the MMP-1 : CGS-27023A complex .
	manualset3
220030	5	420459	7	NULL	NULL	0	NULL	experimental NMR restraints	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The solution structure of the complex was calculated by means of hybrid distance geometry-simulated annealing using a combination of experimental NMR restraints obtained from the previous refinement of the inhibitor-free MMP-1 ( 1 ) and recent restraints for the MMP-1 : CGS-27023A complex .
	manualset3
220031	6	420459	7	NULL	NULL	0	NULL	previous refinement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The solution structure of the complex was calculated by means of hybrid distance geometry-simulated annealing using a combination of experimental NMR restraints obtained from the previous refinement of the inhibitor-free MMP-1 ( 1 ) and recent restraints for the MMP-1 : CGS-27023A complex .
	manualset3
220032	7	420459	7	NULL	NULL	0	NULL	inhibitor-free MMP-1 ( 1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The solution structure of the complex was calculated by means of hybrid distance geometry-simulated annealing using a combination of experimental NMR restraints obtained from the previous refinement of the inhibitor-free MMP-1 ( 1 ) and recent restraints for the MMP-1 : CGS-27023A complex .
	manualset3
220033	8	420459	7	NULL	NULL	0	NULL	restraints	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The solution structure of the complex was calculated by means of hybrid distance geometry-simulated annealing using a combination of experimental NMR restraints obtained from the previous refinement of the inhibitor-free MMP-1 ( 1 ) and recent restraints for the MMP-1 : CGS-27023A complex .
	manualset3
220034	9	420459	7	NULL	NULL	0	NULL	MMP-1 : CGS-27023A complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The solution structure of the complex was calculated by means of hybrid distance geometry-simulated annealing using a combination of experimental NMR restraints obtained from the previous refinement of the inhibitor-free MMP-1 ( 1 ) and recent restraints for the MMP-1 : CGS-27023A complex .
	manualset3
220035	1	420460	7	NULL	NULL	0	NULL	paper 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This paper is an up-to-date review of current literature of the problem , describing age-related changes in the functioning of three major , complementary pathways of signal transduction in murine and human T cell : IP3/Ca2 + / calcineurin , DAG/protein kinase C ( PKC ) and Ras/MAP kinases , discovered so far .
	manualset3
220036	2	420460	7	NULL	NULL	0	NULL	up-to-date review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This paper is an up-to-date review of current literature of the problem , describing age-related changes in the functioning of three major , complementary pathways of signal transduction in murine and human T cell : IP3/Ca2 + / calcineurin , DAG/protein kinase C ( PKC ) and Ras/MAP kinases , discovered so far .
	manualset3
220037	3	420460	7	NULL	NULL	0	NULL	current literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This paper is an up-to-date review of current literature of the problem , describing age-related changes in the functioning of three major , complementary pathways of signal transduction in murine and human T cell : IP3/Ca2 + / calcineurin , DAG/protein kinase C ( PKC ) and Ras/MAP kinases , discovered so far .
	manualset3
220038	4	420460	7	NULL	NULL	0	NULL	problem	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This paper is an up-to-date review of current literature of the problem , describing age-related changes in the functioning of three major , complementary pathways of signal transduction in murine and human T cell : IP3/Ca2 + / calcineurin , DAG/protein kinase C ( PKC ) and Ras/MAP kinases , discovered so far .
	manualset3
220039	5	420460	7	NULL	NULL	0	NULL	age-related changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This paper is an up-to-date review of current literature of the problem , describing age-related changes in the functioning of three major , complementary pathways of signal transduction in murine and human T cell : IP3/Ca2 + / calcineurin , DAG/protein kinase C ( PKC ) and Ras/MAP kinases , discovered so far .
	manualset3
220040	6	420460	7	NULL	NULL	0	NULL	functioning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This paper is an up-to-date review of current literature of the problem , describing age-related changes in the functioning of three major , complementary pathways of signal transduction in murine and human T cell : IP3/Ca2 + / calcineurin , DAG/protein kinase C ( PKC ) and Ras/MAP kinases , discovered so far .
	manualset3
220041	7	420460	7	NULL	NULL	NULL	NULL	three major , complementary pathways	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This paper is an up-to-date review of current literature of the problem , describing age-related changes in the functioning of three major , complementary pathways of signal transduction in murine and human T cell : IP3/Ca2 + / calcineurin , DAG/protein kinase C ( PKC ) and Ras/MAP kinases , discovered so far .
	manualset3
220042	8	420460	7	NULL	NULL	0	NULL	signal transduction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This paper is an up-to-date review of current literature of the problem , describing age-related changes in the functioning of three major , complementary pathways of signal transduction in murine and human T cell : IP3/Ca2 + / calcineurin , DAG/protein kinase C ( PKC ) and Ras/MAP kinases , discovered so far .
	manualset3
220043	9	420460	7	NULL	NULL	0	NULL	murine cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	This paper is an up-to-date review of current literature of the problem , describing age-related changes in the functioning of three major , complementary pathways of signal transduction in murine and human T cell : IP3/Ca2 + / calcineurin , DAG/protein kinase C ( PKC ) and Ras/MAP kinases , discovered so far .
	manualset3
220044	10	420460	7	NULL	NULL	0	NULL	human T cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	This paper is an up-to-date review of current literature of the problem , describing age-related changes in the functioning of three major , complementary pathways of signal transduction in murine and human T cell : IP3/Ca2 + / calcineurin , DAG/protein kinase C ( PKC ) and Ras/MAP kinases , discovered so far .
	manualset3
220045	11	420460	7	NULL	NULL	0	NULL	IP3/Ca2 + / calcineurin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This paper is an up-to-date review of current literature of the problem , describing age-related changes in the functioning of three major , complementary pathways of signal transduction in murine and human T cell : IP3/Ca2 + / calcineurin , DAG/protein kinase C ( PKC ) and Ras/MAP kinases , discovered so far .
	manualset3
220046	12	420460	7	NULL	NULL	0	NULL	DAG/protein kinase C ( PKC )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This paper is an up-to-date review of current literature of the problem , describing age-related changes in the functioning of three major , complementary pathways of signal transduction in murine and human T cell : IP3/Ca2 + / calcineurin , DAG/protein kinase C ( PKC ) and Ras/MAP kinases , discovered so far .
	manualset3
220047	13	420460	7	NULL	NULL	0	NULL	Ras/MAP kinases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This paper is an up-to-date review of current literature of the problem , describing age-related changes in the functioning of three major , complementary pathways of signal transduction in murine and human T cell : IP3/Ca2 + / calcineurin , DAG/protein kinase C ( PKC ) and Ras/MAP kinases , discovered so far .
	manualset3
220048	1	420461	7	NULL	NULL	0	NULL	half 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Over half of all respondents perceived EEE as an equal or greater threat than cancer .
	manualset3
220049	2	420461	7	NULL	NULL	0	NULL	respondents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Over half of all respondents perceived EEE as an equal or greater threat than cancer .
	manualset3
220050	3	420461	7	NULL	NULL	0	NULL	EEE 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Over half of all respondents perceived EEE as an equal or greater threat than cancer .
	manualset3
220051	4	420461	7	NULL	NULL	0	NULL	cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Over half of all respondents perceived EEE as an equal or greater threat than cancer .
	manualset3
220052	1	420462	7	NULL	NULL	0	NULL	Alu-vector PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Alu-vector PCR with biotinylated primers to isolate YAC ends ready for sequencing .
	manualset3
220053	2	420462	7	NULL	NULL	0	NULL	biotinylated primers	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Alu-vector PCR with biotinylated primers to isolate YAC ends ready for sequencing .
	manualset3
220054	3	420462	7	NULL	NULL	0	NULL	YAC ends	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Alu-vector PCR with biotinylated primers to isolate YAC ends ready for sequencing .
	manualset3
220055	4	420462	7	NULL	NULL	0	NULL	sequencing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Alu-vector PCR with biotinylated primers to isolate YAC ends ready for sequencing .
	manualset3
220056	1	420463	7	NULL	NULL	0	NULL	Noninvasive cardioversion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Noninvasive cardioversion of atrial tachycardia using dual-chamber definitive stimulator ) .
	manualset3
220057	2	420463	7	NULL	NULL	0	NULL	atrial tachycardia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Noninvasive cardioversion of atrial tachycardia using dual-chamber definitive stimulator ) .
	manualset3
220058	3	420463	7	NULL	NULL	0	NULL	dual-chamber definitive stimulator	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	( Noninvasive cardioversion of atrial tachycardia using dual-chamber definitive stimulator ) .
	manualset3
220059	1	420464	7	NULL	NULL	0	NULL	carrier mediated T ( 4 ) transport	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This suggests that increased carrier mediated T ( 4 ) transport by placental TTR may be induced by the low oxygen environment of early pregnancy , a time when the fetus has its highest requirement for transport of maternal T ( 4 ) .
	manualset3
220060	2	420464	7	NULL	NULL	0	NULL	 placental TTR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This suggests that increased carrier mediated T ( 4 ) transport by placental TTR may be induced by the low oxygen environment of early pregnancy , a time when the fetus has its highest requirement for transport of maternal T ( 4 ) .
	manualset3
220061	3	420464	7	NULL	NULL	0	NULL	low oxygen environment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This suggests that increased carrier mediated T ( 4 ) transport by placental TTR may be induced by the low oxygen environment of early pregnancy , a time when the fetus has its highest requirement for transport of maternal T ( 4 ) .
	manualset3
220062	4	420464	7	NULL	NULL	0	NULL	early pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This suggests that increased carrier mediated T ( 4 ) transport by placental TTR may be induced by the low oxygen environment of early pregnancy , a time when the fetus has its highest requirement for transport of maternal T ( 4 ) .
	manualset3
220063	5	420464	7	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	This suggests that increased carrier mediated T ( 4 ) transport by placental TTR may be induced by the low oxygen environment of early pregnancy , a time when the fetus has its highest requirement for transport of maternal T ( 4 ) .
	manualset3
220064	6	420464	7	NULL	NULL	0	NULL	fetus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	This suggests that increased carrier mediated T ( 4 ) transport by placental TTR may be induced by the low oxygen environment of early pregnancy , a time when the fetus has its highest requirement for transport of maternal T ( 4 ) .
	manualset3
220065	7	420464	7	NULL	NULL	0	NULL	transport 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This suggests that increased carrier mediated T ( 4 ) transport by placental TTR may be induced by the low oxygen environment of early pregnancy , a time when the fetus has its highest requirement for transport of maternal T ( 4 ) .
	manualset3
220066	8	420464	7	NULL	NULL	NULL	NULL	maternal T ( 4 )	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This suggests that increased carrier mediated T ( 4 ) transport by placental TTR may be induced by the low oxygen environment of early pregnancy , a time when the fetus has its highest requirement for transport of maternal T ( 4 ) .
	manualset3
220067	9	420464	7	NULL	NULL	0	NULL	highest requirement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This suggests that increased carrier mediated T ( 4 ) transport by placental TTR may be induced by the low oxygen environment of early pregnancy , a time when the fetus has its highest requirement for transport of maternal T ( 4 ) .
	manualset3
220068	1	420465	7	NULL	NULL	NULL	NULL	PBK/TOPK	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	PBK/TOPK ( PDZ-binding kinase , T-LAK-cell-originated protein kinase ) is a serine-threonine kinase that is overexpressed in a variety of tumor cells but its role in oncogenesis remains unclear .
	manualset3
220069	2	420465	7	NULL	NULL	0	NULL	PDZ-binding kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PBK/TOPK ( PDZ-binding kinase , T-LAK-cell-originated protein kinase ) is a serine-threonine kinase that is overexpressed in a variety of tumor cells but its role in oncogenesis remains unclear .
	manualset3
220070	3	420465	7	NULL	NULL	0	NULL	T-LAK-cell-originated protein kinase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PBK/TOPK ( PDZ-binding kinase , T-LAK-cell-originated protein kinase ) is a serine-threonine kinase that is overexpressed in a variety of tumor cells but its role in oncogenesis remains unclear .
	manualset3
220071	4	420465	7	NULL	NULL	0	NULL	serine-threonine kinase	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	PBK/TOPK ( PDZ-binding kinase , T-LAK-cell-originated protein kinase ) is a serine-threonine kinase that is overexpressed in a variety of tumor cells but its role in oncogenesis remains unclear .
	manualset3
220073	6	420465	7	NULL	NULL	0	NULL	tumor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	PBK/TOPK ( PDZ-binding kinase , T-LAK-cell-originated protein kinase ) is a serine-threonine kinase that is overexpressed in a variety of tumor cells but its role in oncogenesis remains unclear .
	manualset3
220074	7	420465	7	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PBK/TOPK ( PDZ-binding kinase , T-LAK-cell-originated protein kinase ) is a serine-threonine kinase that is overexpressed in a variety of tumor cells but its role in oncogenesis remains unclear .
	manualset3
220075	8	420465	7	NULL	NULL	0	NULL	oncogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PBK/TOPK ( PDZ-binding kinase , T-LAK-cell-originated protein kinase ) is a serine-threonine kinase that is overexpressed in a variety of tumor cells but its role in oncogenesis remains unclear .
	manualset3
220076	1	420466	7	NULL	NULL	0	NULL	session 2	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	During session 2 , control subjects again did not show a preference for labeled or unlabeled containers .
	manualset3
220077	2	420466	7	NULL	NULL	0	NULL	control subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	During session 2 , control subjects again did not show a preference for labeled or unlabeled containers .
	manualset3
220078	3	420466	7	NULL	NULL	0	NULL	preference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	During session 2 , control subjects again did not show a preference for labeled or unlabeled containers .
	manualset3
220079	4	420466	7	NULL	NULL	0	NULL	labeled containers	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	During session 2 , control subjects again did not show a preference for labeled or unlabeled containers .
	manualset3
220080	5	420466	7	NULL	NULL	0	NULL	unlabeled containers	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	During session 2 , control subjects again did not show a preference for labeled or unlabeled containers .
	manualset3
220081	1	420467	7	NULL	NULL	0	NULL	FF-PE	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate whether FF-PE had a direct effect on producing these non-reproducible bands , 7 gastrectomy samples were prospectively divided into EF and FF-PE halves for IgH PCR .
	manualset3
220082	2	420467	7	NULL	NULL	0	NULL	direct effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate whether FF-PE had a direct effect on producing these non-reproducible bands , 7 gastrectomy samples were prospectively divided into EF and FF-PE halves for IgH PCR .
	manualset3
220083	3	420467	7	NULL	NULL	0	NULL	non-reproducible bands	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate whether FF-PE had a direct effect on producing these non-reproducible bands , 7 gastrectomy samples were prospectively divided into EF and FF-PE halves for IgH PCR .
	manualset3
220084	4	420467	7	NULL	NULL	0	NULL	7 gastrectomy samples 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate whether FF-PE had a direct effect on producing these non-reproducible bands , 7 gastrectomy samples were prospectively divided into EF and FF-PE halves for IgH PCR .
	manualset3
220085	5	420467	7	NULL	NULL	0	NULL	EF halves	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate whether FF-PE had a direct effect on producing these non-reproducible bands , 7 gastrectomy samples were prospectively divided into EF and FF-PE halves for IgH PCR .
	manualset3
220086	6	420467	7	NULL	NULL	0	NULL	FF-PE halves	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate whether FF-PE had a direct effect on producing these non-reproducible bands , 7 gastrectomy samples were prospectively divided into EF and FF-PE halves for IgH PCR .
	manualset3
220087	7	420467	7	NULL	NULL	0	NULL	IgH PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To investigate whether FF-PE had a direct effect on producing these non-reproducible bands , 7 gastrectomy samples were prospectively divided into EF and FF-PE halves for IgH PCR .
	manualset3
220088	1	420468	7	NULL	NULL	0	NULL	interactional complexity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the interactional complexity of living bodies can only be expressed by invoking biological theories .
	manualset3
220089	2	420468	7	NULL	NULL	0	NULL	living bodies	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the interactional complexity of living bodies can only be expressed by invoking biological theories .
	manualset3
220090	3	420468	7	NULL	NULL	0	NULL	biological theories	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the interactional complexity of living bodies can only be expressed by invoking biological theories .
	manualset3
220091	1	420469	7	NULL	NULL	NULL	NULL	Control	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Control of ventricular tachycardia by rapid electric stimulation of the ventricle ) .
	manualset3
220092	2	420469	7	NULL	NULL	NULL	NULL	ventricular tachycardia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Control of ventricular tachycardia by rapid electric stimulation of the ventricle ) .
	manualset3
220093	3	420469	7	NULL	NULL	NULL	NULL	 rapid electric stimulation 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Control of ventricular tachycardia by rapid electric stimulation of the ventricle ) .
	manualset3
220094	4	420469	7	NULL	NULL	0	NULL	ventricle 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Control of ventricular tachycardia by rapid electric stimulation of the ventricle ) .
	manualset3
220095	1	420470	7	NULL	NULL	0	NULL	Diabetes 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Diabetes and advanced glycation endproducts .
	manualset3
220096	2	420470	7	NULL	NULL	0	NULL	advanced glycation endproducts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Diabetes and advanced glycation endproducts .
	manualset3
220097	1	420471	7	NULL	NULL	0	NULL	certification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Getting ready for certification : urolithiasis .
	manualset3
220098	2	420471	7	NULL	NULL	0	NULL	urolithiasis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Getting ready for certification : urolithiasis .
	manualset3
220099	1	420472	7	NULL	NULL	0	NULL	feasibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We investigated the feasibility of delivering exogenous genes into spinal cord using direct in vivo electrotransfection .
	manualset3
220100	2	420472	7	NULL	NULL	0	NULL	exogenous genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We investigated the feasibility of delivering exogenous genes into spinal cord using direct in vivo electrotransfection .
	manualset3
220101	3	420472	7	NULL	NULL	0	NULL	spinal cord	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We investigated the feasibility of delivering exogenous genes into spinal cord using direct in vivo electrotransfection .
	manualset3
220102	4	420472	7	NULL	NULL	NULL	NULL	direct in vivo electrotransfection	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We investigated the feasibility of delivering exogenous genes into spinal cord using direct in vivo electrotransfection .
	manualset3
220103	1	420473	7	NULL	NULL	0	NULL	 no differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , no differences in modification levels were found in either VP0 and VP4 proteins isolated from mature mutant virions , indicating that myristoylation is required for assembly of the infectious virion .
	manualset3
220104	2	420473	7	NULL	NULL	0	NULL	modification levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , no differences in modification levels were found in either VP0 and VP4 proteins isolated from mature mutant virions , indicating that myristoylation is required for assembly of the infectious virion .
	manualset3
220105	3	420473	7	NULL	NULL	0	NULL	VP0 proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , no differences in modification levels were found in either VP0 and VP4 proteins isolated from mature mutant virions , indicating that myristoylation is required for assembly of the infectious virion .
	manualset3
220106	4	420473	7	NULL	NULL	0	NULL	VP4 proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , no differences in modification levels were found in either VP0 and VP4 proteins isolated from mature mutant virions , indicating that myristoylation is required for assembly of the infectious virion .
	manualset3
220107	5	420473	7	NULL	NULL	0	NULL	mature mutant virions 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , no differences in modification levels were found in either VP0 and VP4 proteins isolated from mature mutant virions , indicating that myristoylation is required for assembly of the infectious virion .
	manualset3
220108	6	420473	7	NULL	NULL	0	NULL	myristoylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , no differences in modification levels were found in either VP0 and VP4 proteins isolated from mature mutant virions , indicating that myristoylation is required for assembly of the infectious virion .
	manualset3
220109	7	420473	7	NULL	NULL	0	NULL	assembly	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , no differences in modification levels were found in either VP0 and VP4 proteins isolated from mature mutant virions , indicating that myristoylation is required for assembly of the infectious virion .
	manualset3
220110	8	420473	7	NULL	NULL	0	NULL	infectious virion	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , no differences in modification levels were found in either VP0 and VP4 proteins isolated from mature mutant virions , indicating that myristoylation is required for assembly of the infectious virion .
	manualset3
220111	1	420474	7	NULL	NULL	0	NULL	Aluminum-related osteodystrophy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Aluminum-related osteodystrophy , a crippling disease in patients with renal failure , can develop from the long-term ingestion of aluminum hydroxide gels .
	manualset3
220112	2	420474	7	NULL	NULL	0	NULL	crippling disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Aluminum-related osteodystrophy , a crippling disease in patients with renal failure , can develop from the long-term ingestion of aluminum hydroxide gels .
	manualset3
220113	3	420474	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Aluminum-related osteodystrophy , a crippling disease in patients with renal failure , can develop from the long-term ingestion of aluminum hydroxide gels .
	manualset3
220114	4	420474	7	NULL	NULL	0	NULL	renal failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Aluminum-related osteodystrophy , a crippling disease in patients with renal failure , can develop from the long-term ingestion of aluminum hydroxide gels .
	manualset3
220115	5	420474	7	NULL	NULL	0	NULL	long-term ingestion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Aluminum-related osteodystrophy , a crippling disease in patients with renal failure , can develop from the long-term ingestion of aluminum hydroxide gels .
	manualset3
220116	6	420474	7	NULL	NULL	0	NULL	aluminum hydroxide gels	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Aluminum-related osteodystrophy , a crippling disease in patients with renal failure , can develop from the long-term ingestion of aluminum hydroxide gels .
	manualset3
220117	1	420475	7	NULL	NULL	0	NULL	Cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells lacking these haplotypes and carrying Kk , Kj , Dk , Dj , or Db were resistant , yielding levels of infection below 20 % .
	manualset3
220118	2	420475	7	NULL	NULL	0	NULL	haplotypes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells lacking these haplotypes and carrying Kk , Kj , Dk , Dj , or Db were resistant , yielding levels of infection below 20 % .
	manualset3
220119	3	420475	7	NULL	NULL	0	NULL	Kk	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells lacking these haplotypes and carrying Kk , Kj , Dk , Dj , or Db were resistant , yielding levels of infection below 20 % .
	manualset3
220120	4	420475	7	NULL	NULL	0	NULL	Kj	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells lacking these haplotypes and carrying Kk , Kj , Dk , Dj , or Db were resistant , yielding levels of infection below 20 % .
	manualset3
220121	5	420475	7	NULL	NULL	0	NULL	 Dk	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells lacking these haplotypes and carrying Kk , Kj , Dk , Dj , or Db were resistant , yielding levels of infection below 20 % .
	manualset3
220122	6	420475	7	NULL	NULL	0	NULL	Dj	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells lacking these haplotypes and carrying Kk , Kj , Dk , Dj , or Db were resistant , yielding levels of infection below 20 % .
	manualset3
220123	7	420475	7	NULL	NULL	0	NULL	Db	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells lacking these haplotypes and carrying Kk , Kj , Dk , Dj , or Db were resistant , yielding levels of infection below 20 % .
	manualset3
220124	8	420475	7	NULL	NULL	0	NULL	levels of infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells lacking these haplotypes and carrying Kk , Kj , Dk , Dj , or Db were resistant , yielding levels of infection below 20 % .
	manualset3
220125	9	420475	7	NULL	NULL	0	NULL	20 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells lacking these haplotypes and carrying Kk , Kj , Dk , Dj , or Db were resistant , yielding levels of infection below 20 % .
	manualset3
220126	1	420476	7	NULL	NULL	0	NULL	Mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in a novel gene , VMD2 , encoding a protein of unknown properties cause juvenile-onset vitelliform macular dystrophy ( Best 's disease ) .
	manualset3
220127	2	420476	7	NULL	NULL	0	NULL	novel gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in a novel gene , VMD2 , encoding a protein of unknown properties cause juvenile-onset vitelliform macular dystrophy ( Best 's disease ) .
	manualset3
220128	3	420476	7	NULL	NULL	0	NULL	VMD2	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in a novel gene , VMD2 , encoding a protein of unknown properties cause juvenile-onset vitelliform macular dystrophy ( Best 's disease ) .
	manualset3
220129	4	420476	7	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in a novel gene , VMD2 , encoding a protein of unknown properties cause juvenile-onset vitelliform macular dystrophy ( Best 's disease ) .
	manualset3
220130	5	420476	7	NULL	NULL	0	NULL	unknown properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in a novel gene , VMD2 , encoding a protein of unknown properties cause juvenile-onset vitelliform macular dystrophy ( Best 's disease ) .
	manualset3
220131	6	420476	7	NULL	NULL	0	NULL	juvenile-onset vitelliform macular dystrophy ( Best 's disease )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in a novel gene , VMD2 , encoding a protein of unknown properties cause juvenile-onset vitelliform macular dystrophy ( Best 's disease ) .
	manualset3
220132	1	420477	7	NULL	NULL	0	NULL	cell types	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Many cell types including developing oocytes , fibroblasts , epithelia and neurons use mRNA localization as a means to establish polarity .
	manualset3
220133	2	420477	7	NULL	NULL	0	NULL	developing oocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Many cell types including developing oocytes , fibroblasts , epithelia and neurons use mRNA localization as a means to establish polarity .
	manualset3
220134	3	420477	7	NULL	NULL	0	NULL	fibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Many cell types including developing oocytes , fibroblasts , epithelia and neurons use mRNA localization as a means to establish polarity .
	manualset3
220135	4	420477	7	NULL	NULL	0	NULL	epithelia	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Many cell types including developing oocytes , fibroblasts , epithelia and neurons use mRNA localization as a means to establish polarity .
	manualset3
220136	5	420477	7	NULL	NULL	0	NULL	 neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Many cell types including developing oocytes , fibroblasts , epithelia and neurons use mRNA localization as a means to establish polarity .
	manualset3
220137	6	420477	7	NULL	NULL	NULL	NULL	mRNA localization	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Many cell types including developing oocytes , fibroblasts , epithelia and neurons use mRNA localization as a means to establish polarity .
	manualset3
220138	7	420477	7	NULL	NULL	0	NULL	polarity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many cell types including developing oocytes , fibroblasts , epithelia and neurons use mRNA localization as a means to establish polarity .
	manualset3
220139	1	420478	7	NULL	NULL	0	NULL	Expression analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression analyses indicated that this defensin is expressed constitutively in T. villosa with leaf , stem , root , and seed showing almost similar levels of high expression .
	manualset3
220140	2	420478	7	NULL	NULL	0	NULL	defensin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression analyses indicated that this defensin is expressed constitutively in T. villosa with leaf , stem , root , and seed showing almost similar levels of high expression .
	manualset3
220141	3	420478	7	NULL	NULL	0	NULL	 T. villosa 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression analyses indicated that this defensin is expressed constitutively in T. villosa with leaf , stem , root , and seed showing almost similar levels of high expression .
	manualset3
220142	4	420478	7	NULL	NULL	0	NULL	leaf 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression analyses indicated that this defensin is expressed constitutively in T. villosa with leaf , stem , root , and seed showing almost similar levels of high expression .
	manualset3
220143	5	420478	7	NULL	NULL	0	NULL	stem	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression analyses indicated that this defensin is expressed constitutively in T. villosa with leaf , stem , root , and seed showing almost similar levels of high expression .
	manualset3
220144	6	420478	7	NULL	NULL	0	NULL	root	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression analyses indicated that this defensin is expressed constitutively in T. villosa with leaf , stem , root , and seed showing almost similar levels of high expression .
	manualset3
220145	7	420478	7	NULL	NULL	0	NULL	seed	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression analyses indicated that this defensin is expressed constitutively in T. villosa with leaf , stem , root , and seed showing almost similar levels of high expression .
	manualset3
220146	8	420478	7	NULL	NULL	0	NULL	similar levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression analyses indicated that this defensin is expressed constitutively in T. villosa with leaf , stem , root , and seed showing almost similar levels of high expression .
	manualset3
220147	9	420478	7	NULL	NULL	0	NULL	high expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression analyses indicated that this defensin is expressed constitutively in T. villosa with leaf , stem , root , and seed showing almost similar levels of high expression .
	manualset3
220148	1	420479	7	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of NaHCO3 , the increase in protein tyrosine phosphorylation was delayed for 45 min , and this delay was overcome by the addition of dbcAMP and IBMX .
	manualset3
220149	2	420479	7	NULL	NULL	0	NULL	NaHCO3	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of NaHCO3 , the increase in protein tyrosine phosphorylation was delayed for 45 min , and this delay was overcome by the addition of dbcAMP and IBMX .
	manualset3
220150	3	420479	7	NULL	NULL	0	NULL	increase 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of NaHCO3 , the increase in protein tyrosine phosphorylation was delayed for 45 min , and this delay was overcome by the addition of dbcAMP and IBMX .
	manualset3
220151	4	420479	7	NULL	NULL	0	NULL	 protein tyrosine phosphorylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of NaHCO3 , the increase in protein tyrosine phosphorylation was delayed for 45 min , and this delay was overcome by the addition of dbcAMP and IBMX .
	manualset3
220152	5	420479	7	NULL	NULL	0	NULL	45 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of NaHCO3 , the increase in protein tyrosine phosphorylation was delayed for 45 min , and this delay was overcome by the addition of dbcAMP and IBMX .
	manualset3
220153	6	420479	7	NULL	NULL	0	NULL	 delay	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of NaHCO3 , the increase in protein tyrosine phosphorylation was delayed for 45 min , and this delay was overcome by the addition of dbcAMP and IBMX .
	manualset3
220154	7	420479	7	NULL	NULL	0	NULL	 addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of NaHCO3 , the increase in protein tyrosine phosphorylation was delayed for 45 min , and this delay was overcome by the addition of dbcAMP and IBMX .
	manualset3
220155	8	420479	7	NULL	NULL	0	NULL	dbcAMP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of NaHCO3 , the increase in protein tyrosine phosphorylation was delayed for 45 min , and this delay was overcome by the addition of dbcAMP and IBMX .
	manualset3
220156	9	420479	7	NULL	NULL	0	NULL	IBMX	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the absence of NaHCO3 , the increase in protein tyrosine phosphorylation was delayed for 45 min , and this delay was overcome by the addition of dbcAMP and IBMX .
	manualset3
220157	1	420480	7	NULL	NULL	0	NULL	Presence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Presence of two types of cholinesterase in the thymus of infants ) .
	manualset3
220158	2	420480	7	NULL	NULL	0	NULL	 two types	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Presence of two types of cholinesterase in the thymus of infants ) .
	manualset3
220159	3	420480	7	NULL	NULL	0	NULL	cholinesterase	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Presence of two types of cholinesterase in the thymus of infants ) .
	manualset3
220160	4	420480	7	NULL	NULL	0	NULL	thymus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Presence of two types of cholinesterase in the thymus of infants ) .
	manualset3
220161	5	420480	7	NULL	NULL	0	NULL	infants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Presence of two types of cholinesterase in the thymus of infants ) .
	manualset3
220175	1	420481	7	NULL	NULL	0	NULL	CHRONAXY	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( ON CHRONAXY OF THE LABYRINTHINE SYSTEM OF THE RABBIT UNDER THE INFLUENCE OF CHANGES IN SEROTONIN LEVEL IN THE BRAIN ) .
	manualset3
220176	2	420481	7	NULL	NULL	0	NULL	LABYRINTHINE SYSTEM	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( ON CHRONAXY OF THE LABYRINTHINE SYSTEM OF THE RABBIT UNDER THE INFLUENCE OF CHANGES IN SEROTONIN LEVEL IN THE BRAIN ) .
	manualset3
220177	3	420481	7	NULL	NULL	0	NULL	RABBIT 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( ON CHRONAXY OF THE LABYRINTHINE SYSTEM OF THE RABBIT UNDER THE INFLUENCE OF CHANGES IN SEROTONIN LEVEL IN THE BRAIN ) .
	manualset3
220178	4	420481	7	NULL	NULL	0	NULL	 INFLUENCE	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( ON CHRONAXY OF THE LABYRINTHINE SYSTEM OF THE RABBIT UNDER THE INFLUENCE OF CHANGES IN SEROTONIN LEVEL IN THE BRAIN ) .
	manualset3
220179	5	420481	7	NULL	NULL	0	NULL	CHANGES	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( ON CHRONAXY OF THE LABYRINTHINE SYSTEM OF THE RABBIT UNDER THE INFLUENCE OF CHANGES IN SEROTONIN LEVEL IN THE BRAIN ) .
	manualset3
220180	6	420481	7	NULL	NULL	0	NULL	SEROTONIN LEVEL	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( ON CHRONAXY OF THE LABYRINTHINE SYSTEM OF THE RABBIT UNDER THE INFLUENCE OF CHANGES IN SEROTONIN LEVEL IN THE BRAIN ) .
	manualset3
220181	7	420481	7	NULL	NULL	0	NULL	BRAIN	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( ON CHRONAXY OF THE LABYRINTHINE SYSTEM OF THE RABBIT UNDER THE INFLUENCE OF CHANGES IN SEROTONIN LEVEL IN THE BRAIN ) .
	manualset3
220182	1	420482	7	NULL	NULL	0	NULL	molecular weight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weight of the enzyme was estimated by sucrose gradient centrifugation and gel filtrations on Sephadex G-100 to be approximately 63 , 000 to 68 , 000 .
	manualset3
220183	2	420482	7	NULL	NULL	0	NULL	enzyme	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weight of the enzyme was estimated by sucrose gradient centrifugation and gel filtrations on Sephadex G-100 to be approximately 63 , 000 to 68 , 000 .
	manualset3
220184	3	420482	7	NULL	NULL	0	NULL	sucrose gradient centrifugation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weight of the enzyme was estimated by sucrose gradient centrifugation and gel filtrations on Sephadex G-100 to be approximately 63 , 000 to 68 , 000 .
	manualset3
220185	4	420482	7	NULL	NULL	0	NULL	gel filtrations 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weight of the enzyme was estimated by sucrose gradient centrifugation and gel filtrations on Sephadex G-100 to be approximately 63 , 000 to 68 , 000 .
	manualset3
220186	5	420482	7	NULL	NULL	0	NULL	Sephadex G-100	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weight of the enzyme was estimated by sucrose gradient centrifugation and gel filtrations on Sephadex G-100 to be approximately 63 , 000 to 68 , 000 .
	manualset3
220187	6	420482	7	NULL	NULL	0	NULL	63 , 000	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weight of the enzyme was estimated by sucrose gradient centrifugation and gel filtrations on Sephadex G-100 to be approximately 63 , 000 to 68 , 000 .
	manualset3
220188	7	420482	7	NULL	NULL	0	NULL	68 , 000	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular weight of the enzyme was estimated by sucrose gradient centrifugation and gel filtrations on Sephadex G-100 to be approximately 63 , 000 to 68 , 000 .
	manualset3
220189	1	420483	7	NULL	NULL	0	NULL	Alveolar soft part sarcoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Alveolar soft part sarcoma : review of nine cases including two cases with unusual histology .
	manualset3
220190	2	420483	7	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Alveolar soft part sarcoma : review of nine cases including two cases with unusual histology .
	manualset3
220191	3	420483	7	NULL	NULL	0	NULL	nine cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Alveolar soft part sarcoma : review of nine cases including two cases with unusual histology .
	manualset3
220192	4	420483	7	NULL	NULL	0	NULL	two cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Alveolar soft part sarcoma : review of nine cases including two cases with unusual histology .
	manualset3
220193	5	420483	7	NULL	NULL	0	NULL	unusual histology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Alveolar soft part sarcoma : review of nine cases including two cases with unusual histology .
	manualset3
220194	1	420484	7	NULL	NULL	0	NULL	CLO	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	After CLO , sows engaged in nest-building more during Hours 32-17 and less during Hours 16-0 .
	manualset3
220195	2	420484	7	NULL	NULL	0	NULL	sows	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	After CLO , sows engaged in nest-building more during Hours 32-17 and less during Hours 16-0 .
	manualset3
220196	3	420484	7	NULL	NULL	0	NULL	nest-building	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After CLO , sows engaged in nest-building more during Hours 32-17 and less during Hours 16-0 .
	manualset3
220197	4	420484	7	NULL	NULL	0	NULL	Hours 32-17	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After CLO , sows engaged in nest-building more during Hours 32-17 and less during Hours 16-0 .
	manualset3
220198	5	420484	7	NULL	NULL	0	NULL	Hours 16-0	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After CLO , sows engaged in nest-building more during Hours 32-17 and less during Hours 16-0 .
	manualset3
220199	1	420485	7	NULL	NULL	0	NULL	 improved procedure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An improved procedure for the purification of a lipid-containing acidophilic thermophilic bacteriophage , phiNS11 , is described .
	manualset3
220200	2	420485	7	NULL	NULL	0	NULL	 purification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An improved procedure for the purification of a lipid-containing acidophilic thermophilic bacteriophage , phiNS11 , is described .
	manualset3
220201	3	420485	7	NULL	NULL	0	NULL	lipid-containing acidophilic thermophilic bacteriophage 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	An improved procedure for the purification of a lipid-containing acidophilic thermophilic bacteriophage , phiNS11 , is described .
	manualset3
220202	4	420485	7	NULL	NULL	0	NULL	phiNS11 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	An improved procedure for the purification of a lipid-containing acidophilic thermophilic bacteriophage , phiNS11 , is described .
	manualset3
220203	1	420486	7	NULL	NULL	0	NULL	Group 1 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 1 consisting of 12 patients over 70 years of age , and Group 2 consisting of 22 patients under 69 years of age were compared .
	manualset3
220204	2	420486	7	NULL	NULL	0	NULL	12 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 1 consisting of 12 patients over 70 years of age , and Group 2 consisting of 22 patients under 69 years of age were compared .
	manualset3
220205	3	420486	7	NULL	NULL	0	NULL	70 years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 1 consisting of 12 patients over 70 years of age , and Group 2 consisting of 22 patients under 69 years of age were compared .
	manualset3
220206	4	420486	7	NULL	NULL	0	NULL	age	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 1 consisting of 12 patients over 70 years of age , and Group 2 consisting of 22 patients under 69 years of age were compared .
	manualset3
220207	5	420486	7	NULL	NULL	0	NULL	Group 2	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 1 consisting of 12 patients over 70 years of age , and Group 2 consisting of 22 patients under 69 years of age were compared .
	manualset3
220208	6	420486	7	NULL	NULL	0	NULL	22 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 1 consisting of 12 patients over 70 years of age , and Group 2 consisting of 22 patients under 69 years of age were compared .
	manualset3
220209	7	420486	7	NULL	NULL	0	NULL	69 years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 1 consisting of 12 patients over 70 years of age , and Group 2 consisting of 22 patients under 69 years of age were compared .
	manualset3
220210	8	420486	7	NULL	NULL	0	NULL	age 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 1 consisting of 12 patients over 70 years of age , and Group 2 consisting of 22 patients under 69 years of age were compared .
	manualset3
220211	1	420487	7	NULL	NULL	0	NULL	Spleen cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Spleen cells from the immunized mice showed strong cytotoxic activity against E.G7-OVA cells , but not against the parental EL4 cells .
	manualset3
220212	2	420487	7	NULL	NULL	0	NULL	immunized mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Spleen cells from the immunized mice showed strong cytotoxic activity against E.G7-OVA cells , but not against the parental EL4 cells .
	manualset3
220213	3	420487	7	NULL	NULL	0	NULL	cytotoxic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Spleen cells from the immunized mice showed strong cytotoxic activity against E.G7-OVA cells , but not against the parental EL4 cells .
	manualset3
220214	4	420487	7	NULL	NULL	0	NULL	E.G7-OVA cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Spleen cells from the immunized mice showed strong cytotoxic activity against E.G7-OVA cells , but not against the parental EL4 cells .
	manualset3
220215	5	420487	7	NULL	NULL	0	NULL	 parental EL4 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Spleen cells from the immunized mice showed strong cytotoxic activity against E.G7-OVA cells , but not against the parental EL4 cells .
	manualset3
220216	1	420488	7	NULL	NULL	0	NULL	 anisakis body 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The anisakis body was found in the submucosal layer of the resection specimen .
	manualset3
220217	2	420488	7	NULL	NULL	0	NULL	submucosal layer 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The anisakis body was found in the submucosal layer of the resection specimen .
	manualset3
220218	3	420488	7	NULL	NULL	0	NULL	 resection specimen	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The anisakis body was found in the submucosal layer of the resection specimen .
	manualset3
220219	1	420489	7	NULL	NULL	0	NULL	fetal period 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	First , in the fetal period , intravaginal echocardiography allows earlier diagnosis of significant cardiac abnormalities that could lead to a wanted termination of pregnancy .
	manualset3
220220	2	420489	7	NULL	NULL	0	NULL	intravaginal echocardiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	First , in the fetal period , intravaginal echocardiography allows earlier diagnosis of significant cardiac abnormalities that could lead to a wanted termination of pregnancy .
	manualset3
220221	3	420489	7	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	First , in the fetal period , intravaginal echocardiography allows earlier diagnosis of significant cardiac abnormalities that could lead to a wanted termination of pregnancy .
	manualset3
220222	4	420489	7	NULL	NULL	0	NULL	cardiac abnormalities 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	First , in the fetal period , intravaginal echocardiography allows earlier diagnosis of significant cardiac abnormalities that could lead to a wanted termination of pregnancy .
	manualset3
220223	5	420489	7	NULL	NULL	0	NULL	termination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	First , in the fetal period , intravaginal echocardiography allows earlier diagnosis of significant cardiac abnormalities that could lead to a wanted termination of pregnancy .
	manualset3
220224	6	420489	7	NULL	NULL	0	NULL	pregnancy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	First , in the fetal period , intravaginal echocardiography allows earlier diagnosis of significant cardiac abnormalities that could lead to a wanted termination of pregnancy .
	manualset3
220225	1	420490	7	NULL	NULL	0	NULL	Knowledge	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Knowledge of pollution history seems therefore to be of primary importance .
	manualset3
220226	2	420490	7	NULL	NULL	0	NULL	pollution history 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Knowledge of pollution history seems therefore to be of primary importance .
	manualset3
220227	1	420491	7	NULL	NULL	0	NULL	Alzheimer 's disease ( AD ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Alzheimer 's disease ( AD ) remains a major health problem , and accounts for 50 to 60 % of all cases of dementia .
	manualset3
220228	2	420491	7	NULL	NULL	0	NULL	major health problem 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Alzheimer 's disease ( AD ) remains a major health problem , and accounts for 50 to 60 % of all cases of dementia .
	manualset3
220229	3	420491	7	NULL	NULL	0	NULL	 50%	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Alzheimer 's disease ( AD ) remains a major health problem , and accounts for 50 to 60 % of all cases of dementia .
	manualset3
220230	4	420491	7	NULL	NULL	0	NULL	 60%	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Alzheimer 's disease ( AD ) remains a major health problem , and accounts for 50 to 60 % of all cases of dementia .
	manualset3
220231	5	420491	7	NULL	NULL	0	NULL	cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Alzheimer 's disease ( AD ) remains a major health problem , and accounts for 50 to 60 % of all cases of dementia .
	manualset3
220232	6	420491	7	NULL	NULL	0	NULL	dementia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Alzheimer 's disease ( AD ) remains a major health problem , and accounts for 50 to 60 % of all cases of dementia .
	manualset3
220233	1	420492	7	NULL	NULL	0	NULL	Limiting dilution analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Limiting dilution analysis indicated that the vast majority ( ) 90 % ) of VSV pCTL failed to become primed when exposed to VSV in the absence of CD4 + cells .
	manualset3
220234	2	420492	7	NULL	NULL	0	NULL	majority	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Limiting dilution analysis indicated that the vast majority ( ) 90 % ) of VSV pCTL failed to become primed when exposed to VSV in the absence of CD4 + cells .
	manualset3
220235	3	420492	7	NULL	NULL	0	NULL	90 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Limiting dilution analysis indicated that the vast majority ( ) 90 % ) of VSV pCTL failed to become primed when exposed to VSV in the absence of CD4 + cells .
	manualset3
220236	4	420492	7	NULL	NULL	0	NULL	VSV pCTL	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Limiting dilution analysis indicated that the vast majority ( ) 90 % ) of VSV pCTL failed to become primed when exposed to VSV in the absence of CD4 + cells .
	manualset3
220237	5	420492	7	NULL	NULL	0	NULL	VSV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Limiting dilution analysis indicated that the vast majority ( ) 90 % ) of VSV pCTL failed to become primed when exposed to VSV in the absence of CD4 + cells .
	manualset3
220238	6	420492	7	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Limiting dilution analysis indicated that the vast majority ( ) 90 % ) of VSV pCTL failed to become primed when exposed to VSV in the absence of CD4 + cells .
	manualset3
220239	7	420492	7	NULL	NULL	0	NULL	CD4 + cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Limiting dilution analysis indicated that the vast majority ( ) 90 % ) of VSV pCTL failed to become primed when exposed to VSV in the absence of CD4 + cells .
	manualset3
220240	1	420493	7	NULL	NULL	0	NULL	Analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of raft affinity of membrane proteins by detergent-insolubility .
	manualset3
220241	2	420493	7	NULL	NULL	0	NULL	 raft affinity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of raft affinity of membrane proteins by detergent-insolubility .
	manualset3
220242	3	420493	7	NULL	NULL	0	NULL	membrane proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of raft affinity of membrane proteins by detergent-insolubility .
	manualset3
220243	4	420493	7	NULL	NULL	0	NULL	detergent-insolubility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of raft affinity of membrane proteins by detergent-insolubility .
	manualset3
220244	1	420494	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of mammalian DNA replication lagged behind that of prokaryotes for many years .
	manualset3
220245	2	420494	7	NULL	NULL	0	NULL	mammalian DNA replication	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of mammalian DNA replication lagged behind that of prokaryotes for many years .
	manualset3
220246	3	420494	7	NULL	NULL	0	NULL	prokaryotes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of mammalian DNA replication lagged behind that of prokaryotes for many years .
	manualset3
220247	4	420494	7	NULL	NULL	0	NULL	 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The study of mammalian DNA replication lagged behind that of prokaryotes for many years .
	manualset3
220248	1	420495	7	NULL	NULL	NULL	NULL	patient	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The patient remains in good state of health , 20 months after the procedure .
	manualset3
220249	2	420495	7	NULL	NULL	0	NULL	good state 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient remains in good state of health , 20 months after the procedure .
	manualset3
220250	3	420495	7	NULL	NULL	0	NULL	health 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient remains in good state of health , 20 months after the procedure .
	manualset3
220251	4	420495	7	NULL	NULL	0	NULL	20 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient remains in good state of health , 20 months after the procedure .
	manualset3
220252	5	420495	7	NULL	NULL	0	NULL	procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient remains in good state of health , 20 months after the procedure .
	manualset3
220253	1	420496	7	NULL	NULL	0	NULL	amrinone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	We believe that , when using amrinone to facilitate separation from CPB , a bolus dose of 1.5 mg kg-1 or more should be administered .
	manualset3
220254	2	420496	7	NULL	NULL	0	NULL	separation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We believe that , when using amrinone to facilitate separation from CPB , a bolus dose of 1.5 mg kg-1 or more should be administered .
	manualset3
220255	3	420496	7	NULL	NULL	0	NULL	CPB 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	We believe that , when using amrinone to facilitate separation from CPB , a bolus dose of 1.5 mg kg-1 or more should be administered .
	manualset3
220256	4	420496	7	NULL	NULL	0	NULL	bolus dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We believe that , when using amrinone to facilitate separation from CPB , a bolus dose of 1.5 mg kg-1 or more should be administered .
	manualset3
220257	5	420496	7	NULL	NULL	0	NULL	1.5 mg kg-1	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We believe that , when using amrinone to facilitate separation from CPB , a bolus dose of 1.5 mg kg-1 or more should be administered .
	manualset3
220258	1	420497	7	NULL	NULL	0	NULL	features	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Other features are specific to widowhood , including remarriage , issues of personal autonomy , and loss of status , access to productive resources and social support .
	manualset3
220259	2	420497	7	NULL	NULL	0	NULL	widowhood	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Other features are specific to widowhood , including remarriage , issues of personal autonomy , and loss of status , access to productive resources and social support .
	manualset3
220260	3	420497	7	NULL	NULL	0	NULL	remarriage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Other features are specific to widowhood , including remarriage , issues of personal autonomy , and loss of status , access to productive resources and social support .
	manualset3
220261	4	420497	7	NULL	NULL	0	NULL	issues	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Other features are specific to widowhood , including remarriage , issues of personal autonomy , and loss of status , access to productive resources and social support .
	manualset3
220262	5	420497	7	NULL	NULL	0	NULL	personal autonomy 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Other features are specific to widowhood , including remarriage , issues of personal autonomy , and loss of status , access to productive resources and social support .
	manualset3
220263	6	420497	7	NULL	NULL	0	NULL	loss of status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Other features are specific to widowhood , including remarriage , issues of personal autonomy , and loss of status , access to productive resources and social support .
	manualset3
220264	7	420497	7	NULL	NULL	0	NULL	 productive resources 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Other features are specific to widowhood , including remarriage , issues of personal autonomy , and loss of status , access to productive resources and social support .
	manualset3
220265	8	420497	7	NULL	NULL	0	NULL	social support	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Other features are specific to widowhood , including remarriage , issues of personal autonomy , and loss of status , access to productive resources and social support .
	manualset3
220266	1	420498	7	NULL	NULL	0	NULL	Amadori-modified glycated albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Amadori-modified glycated albumin predominantly induces E-selectin expression on human umbilical vein endothelial cells through NADPH oxidase activation .
	manualset3
220267	2	420498	7	NULL	NULL	0	NULL	E-selectin expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Amadori-modified glycated albumin predominantly induces E-selectin expression on human umbilical vein endothelial cells through NADPH oxidase activation .
	manualset3
220268	3	420498	7	NULL	NULL	0	NULL	human umbilical vein endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Amadori-modified glycated albumin predominantly induces E-selectin expression on human umbilical vein endothelial cells through NADPH oxidase activation .
	manualset3
220269	4	420498	7	NULL	NULL	0	NULL	NADPH oxidase activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Amadori-modified glycated albumin predominantly induces E-selectin expression on human umbilical vein endothelial cells through NADPH oxidase activation .
	manualset3
220270	1	420499	7	NULL	NULL	0	NULL	expression levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the expression levels of TFAM in the IVG oocytes was significantly lower than that of ovulated oocytes and oocytes recovered from follicles with diameters of more than 300 microm .
	manualset3
220271	2	420499	7	NULL	NULL	0	NULL	TFAM	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the expression levels of TFAM in the IVG oocytes was significantly lower than that of ovulated oocytes and oocytes recovered from follicles with diameters of more than 300 microm .
	manualset3
220272	3	420499	7	NULL	NULL	0	NULL	IVG oocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the expression levels of TFAM in the IVG oocytes was significantly lower than that of ovulated oocytes and oocytes recovered from follicles with diameters of more than 300 microm .
	manualset3
220273	4	420499	7	NULL	NULL	0	NULL	ovulated oocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the expression levels of TFAM in the IVG oocytes was significantly lower than that of ovulated oocytes and oocytes recovered from follicles with diameters of more than 300 microm .
	manualset3
220274	5	420499	7	NULL	NULL	0	NULL	 oocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the expression levels of TFAM in the IVG oocytes was significantly lower than that of ovulated oocytes and oocytes recovered from follicles with diameters of more than 300 microm .
	manualset3
220275	6	420499	7	NULL	NULL	0	NULL	follicles 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the expression levels of TFAM in the IVG oocytes was significantly lower than that of ovulated oocytes and oocytes recovered from follicles with diameters of more than 300 microm .
	manualset3
220276	7	420499	7	NULL	NULL	0	NULL	 diameters	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the expression levels of TFAM in the IVG oocytes was significantly lower than that of ovulated oocytes and oocytes recovered from follicles with diameters of more than 300 microm .
	manualset3
220277	8	420499	7	NULL	NULL	0	NULL	300 microm	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the expression levels of TFAM in the IVG oocytes was significantly lower than that of ovulated oocytes and oocytes recovered from follicles with diameters of more than 300 microm .
	manualset3
220278	1	420500	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , a comparative pharmacokinetic study of 2 docetaxel parenteral solutions , SID530 and Taxotere , was carried out .
	manualset3
220279	2	420500	7	NULL	NULL	0	NULL	comparative pharmacokinetic study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , a comparative pharmacokinetic study of 2 docetaxel parenteral solutions , SID530 and Taxotere , was carried out .
	manualset3
220280	3	420500	7	NULL	NULL	0	NULL	2 docetaxel parenteral solutions 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , a comparative pharmacokinetic study of 2 docetaxel parenteral solutions , SID530 and Taxotere , was carried out .
	manualset3
220281	4	420500	7	NULL	NULL	0	NULL	SID530	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , a comparative pharmacokinetic study of 2 docetaxel parenteral solutions , SID530 and Taxotere , was carried out .
	manualset3
220282	5	420500	7	NULL	NULL	0	NULL	Taxotere	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , a comparative pharmacokinetic study of 2 docetaxel parenteral solutions , SID530 and Taxotere , was carried out .
	manualset3
220283	1	420501	7	NULL	NULL	0	NULL	contributions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We discuss possible contributions from other effects that are not related to parity violation .
	manualset3
220284	2	420501	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We discuss possible contributions from other effects that are not related to parity violation .
	manualset3
220285	3	420501	7	NULL	NULL	0	NULL	parity violation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We discuss possible contributions from other effects that are not related to parity violation .
	manualset3
220286	1	420502	7	NULL	NULL	0	NULL	Analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analyses of variance across ethnic categories and chi2 analysis of differences in ethnic group composition between clusters of scales were conducted .
	manualset3
220287	2	420502	7	NULL	NULL	0	NULL	variance	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Analyses of variance across ethnic categories and chi2 analysis of differences in ethnic group composition between clusters of scales were conducted .
	manualset3
220288	3	420502	7	NULL	NULL	0	NULL	ethnic categories 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Analyses of variance across ethnic categories and chi2 analysis of differences in ethnic group composition between clusters of scales were conducted .
	manualset3
220289	4	420502	7	NULL	NULL	0	NULL	chi2 analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analyses of variance across ethnic categories and chi2 analysis of differences in ethnic group composition between clusters of scales were conducted .
	manualset3
220290	5	420502	7	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Analyses of variance across ethnic categories and chi2 analysis of differences in ethnic group composition between clusters of scales were conducted .
	manualset3
220291	6	420502	7	NULL	NULL	0	NULL	ethnic group composition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Analyses of variance across ethnic categories and chi2 analysis of differences in ethnic group composition between clusters of scales were conducted .
	manualset3
220292	7	420502	7	NULL	NULL	0	NULL	clusters of scales	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analyses of variance across ethnic categories and chi2 analysis of differences in ethnic group composition between clusters of scales were conducted .
	manualset3
220293	1	420503	7	NULL	NULL	0	NULL	 frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of MTHFR 677T was found to be 34.3 % .
	manualset3
220294	2	420503	7	NULL	NULL	0	NULL	MTHFR 677T	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of MTHFR 677T was found to be 34.3 % .
	manualset3
220295	3	420503	7	NULL	NULL	0	NULL	34.3 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of MTHFR 677T was found to be 34.3 % .
	manualset3
220296	1	420504	7	NULL	NULL	0	NULL	Amalgam repair 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Amalgam repair : quantitative evaluation of amalgam-resin and resin-tooth interfaces with different surface treatments .
	manualset3
220297	2	420504	7	NULL	NULL	0	NULL	quantitative evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Amalgam repair : quantitative evaluation of amalgam-resin and resin-tooth interfaces with different surface treatments .
	manualset3
220298	3	420504	7	NULL	NULL	0	NULL	amalgam-resin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Amalgam repair : quantitative evaluation of amalgam-resin and resin-tooth interfaces with different surface treatments .
	manualset3
220299	4	420504	7	NULL	NULL	0	NULL	resin-tooth interfaces	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Amalgam repair : quantitative evaluation of amalgam-resin and resin-tooth interfaces with different surface treatments .
	manualset3
220300	5	420504	7	NULL	NULL	0	NULL	surface treatments 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Amalgam repair : quantitative evaluation of amalgam-resin and resin-tooth interfaces with different surface treatments .
	manualset3
220301	1	420505	7	NULL	NULL	0	NULL	Extraction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Extraction of GAG from neonatal rat cartilage with guanidine hydrochloride removes stainable extracellular matrix but not the interlacunar network .
	manualset3
220302	2	420505	7	NULL	NULL	0	NULL	GAG	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Extraction of GAG from neonatal rat cartilage with guanidine hydrochloride removes stainable extracellular matrix but not the interlacunar network .
	manualset3
220303	3	420505	7	NULL	NULL	0	NULL	neonatal rat cartilage	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Extraction of GAG from neonatal rat cartilage with guanidine hydrochloride removes stainable extracellular matrix but not the interlacunar network .
	manualset3
220304	4	420505	7	NULL	NULL	0	NULL	guanidine hydrochloride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Extraction of GAG from neonatal rat cartilage with guanidine hydrochloride removes stainable extracellular matrix but not the interlacunar network .
	manualset3
220305	5	420505	7	NULL	NULL	0	NULL	stainable extracellular matrix	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Extraction of GAG from neonatal rat cartilage with guanidine hydrochloride removes stainable extracellular matrix but not the interlacunar network .
	manualset3
220306	6	420505	7	NULL	NULL	0	NULL	interlacunar network 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Extraction of GAG from neonatal rat cartilage with guanidine hydrochloride removes stainable extracellular matrix but not the interlacunar network .
	manualset3
220307	1	420506	7	NULL	NULL	0	NULL	Astrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Astrocytes exposed to CM-A induced permeabilization of cortical neurons through activation of neuronal pannexin 1 ( Panx1 ) hemichannels by ATP and glutamate released through astroglial Cx43 hemichannels .
	manualset3
220308	2	420506	7	NULL	NULL	0	NULL	CM-A induced permeabilization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Astrocytes exposed to CM-A induced permeabilization of cortical neurons through activation of neuronal pannexin 1 ( Panx1 ) hemichannels by ATP and glutamate released through astroglial Cx43 hemichannels .
	manualset3
220309	3	420506	7	NULL	NULL	0	NULL	cortical neurons	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Astrocytes exposed to CM-A induced permeabilization of cortical neurons through activation of neuronal pannexin 1 ( Panx1 ) hemichannels by ATP and glutamate released through astroglial Cx43 hemichannels .
	manualset3
220310	4	420506	7	NULL	NULL	0	NULL	activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Astrocytes exposed to CM-A induced permeabilization of cortical neurons through activation of neuronal pannexin 1 ( Panx1 ) hemichannels by ATP and glutamate released through astroglial Cx43 hemichannels .
	manualset3
220311	5	420506	7	NULL	NULL	0	NULL	neuronal pannexin 1 ( Panx1 ) hemichannels 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Astrocytes exposed to CM-A induced permeabilization of cortical neurons through activation of neuronal pannexin 1 ( Panx1 ) hemichannels by ATP and glutamate released through astroglial Cx43 hemichannels .
	manualset3
220312	6	420506	7	NULL	NULL	0	NULL	ATP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Astrocytes exposed to CM-A induced permeabilization of cortical neurons through activation of neuronal pannexin 1 ( Panx1 ) hemichannels by ATP and glutamate released through astroglial Cx43 hemichannels .
	manualset3
220313	7	420506	7	NULL	NULL	0	NULL	glutamate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Astrocytes exposed to CM-A induced permeabilization of cortical neurons through activation of neuronal pannexin 1 ( Panx1 ) hemichannels by ATP and glutamate released through astroglial Cx43 hemichannels .
	manualset3
220314	8	420506	7	NULL	NULL	0	NULL	astroglial Cx43 hemichannels 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Astrocytes exposed to CM-A induced permeabilization of cortical neurons through activation of neuronal pannexin 1 ( Panx1 ) hemichannels by ATP and glutamate released through astroglial Cx43 hemichannels .
	manualset3
220315	1	420507	7	NULL	NULL	0	NULL	chromatographic examination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The chromatographic examination of Adonis vernalis L. II .
	manualset3
220316	2	420507	7	NULL	NULL	0	NULL	Adonis vernalis L. II	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The chromatographic examination of Adonis vernalis L. II .
	manualset3
220317	1	420508	7	NULL	NULL	0	NULL	 later times	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	At later times , toxin expression is followed by death of a small fraction ( 10 % ) of PI stained cells that exited earlier or did not enter into the dormant state .
	manualset3
220318	2	420508	7	NULL	NULL	0	NULL	toxin expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	At later times , toxin expression is followed by death of a small fraction ( 10 % ) of PI stained cells that exited earlier or did not enter into the dormant state .
	manualset3
220319	3	420508	7	NULL	NULL	NULL	NULL	death	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At later times , toxin expression is followed by death of a small fraction ( 10 % ) of PI stained cells that exited earlier or did not enter into the dormant state .
	manualset3
220320	4	420508	7	NULL	NULL	0	NULL	small fraction	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	At later times , toxin expression is followed by death of a small fraction ( 10 % ) of PI stained cells that exited earlier or did not enter into the dormant state .
	manualset3
220321	5	420508	7	NULL	NULL	0	NULL	10 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	At later times , toxin expression is followed by death of a small fraction ( 10 % ) of PI stained cells that exited earlier or did not enter into the dormant state .
	manualset3
220322	6	420508	7	NULL	NULL	0	NULL	PI stained cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	At later times , toxin expression is followed by death of a small fraction ( 10 % ) of PI stained cells that exited earlier or did not enter into the dormant state .
	manualset3
220323	7	420508	7	NULL	NULL	0	NULL	dormant state	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	At later times , toxin expression is followed by death of a small fraction ( 10 % ) of PI stained cells that exited earlier or did not enter into the dormant state .
	manualset3
220324	1	420509	7	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	They also revealed that there is no appreciable difference in AcP and betaG activity between B and T lymphocytes obtained from the blood of normal donors .
	manualset3
220325	2	420509	7	NULL	NULL	0	NULL	AcP activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They also revealed that there is no appreciable difference in AcP and betaG activity between B and T lymphocytes obtained from the blood of normal donors .
	manualset3
220326	3	420509	7	NULL	NULL	0	NULL	betaG activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They also revealed that there is no appreciable difference in AcP and betaG activity between B and T lymphocytes obtained from the blood of normal donors .
	manualset3
220327	4	420509	7	NULL	NULL	0	NULL	B lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	They also revealed that there is no appreciable difference in AcP and betaG activity between B and T lymphocytes obtained from the blood of normal donors .
	manualset3
220328	5	420509	7	NULL	NULL	0	NULL	T lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	They also revealed that there is no appreciable difference in AcP and betaG activity between B and T lymphocytes obtained from the blood of normal donors .
	manualset3
220329	6	420509	7	NULL	NULL	0	NULL	blood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	They also revealed that there is no appreciable difference in AcP and betaG activity between B and T lymphocytes obtained from the blood of normal donors .
	manualset3
220330	7	420509	7	NULL	NULL	0	NULL	normal donors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	They also revealed that there is no appreciable difference in AcP and betaG activity between B and T lymphocytes obtained from the blood of normal donors .
	manualset3
220331	1	420510	7	NULL	NULL	0	NULL	Progressive disability 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Progressive disability can be delayed through a variety of physiatric and orthopedic techniques , including surgical release of lower-extremity contracture , repair of foot and ankle deformity , and correction of scoliosis .
	manualset3
220332	2	420510	7	NULL	NULL	NULL	NULL	 physiatric techniques	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Progressive disability can be delayed through a variety of physiatric and orthopedic techniques , including surgical release of lower-extremity contracture , repair of foot and ankle deformity , and correction of scoliosis .
	manualset3
220333	3	420510	7	NULL	NULL	0	NULL	orthopedic techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Progressive disability can be delayed through a variety of physiatric and orthopedic techniques , including surgical release of lower-extremity contracture , repair of foot and ankle deformity , and correction of scoliosis .
	manualset3
220334	4	420510	7	NULL	NULL	0	NULL	surgical release	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Progressive disability can be delayed through a variety of physiatric and orthopedic techniques , including surgical release of lower-extremity contracture , repair of foot and ankle deformity , and correction of scoliosis .
	manualset3
220335	5	420510	7	NULL	NULL	0	NULL	lower-extremity contracture	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Progressive disability can be delayed through a variety of physiatric and orthopedic techniques , including surgical release of lower-extremity contracture , repair of foot and ankle deformity , and correction of scoliosis .
	manualset3
220336	6	420510	7	NULL	NULL	0	NULL	repair	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Progressive disability can be delayed through a variety of physiatric and orthopedic techniques , including surgical release of lower-extremity contracture , repair of foot and ankle deformity , and correction of scoliosis .
	manualset3
220337	7	420510	7	NULL	NULL	0	NULL	foot deformity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Progressive disability can be delayed through a variety of physiatric and orthopedic techniques , including surgical release of lower-extremity contracture , repair of foot and ankle deformity , and correction of scoliosis .
	manualset3
220338	8	420510	7	NULL	NULL	0	NULL	 ankle deformity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Progressive disability can be delayed through a variety of physiatric and orthopedic techniques , including surgical release of lower-extremity contracture , repair of foot and ankle deformity , and correction of scoliosis .
	manualset3
220339	9	420510	7	NULL	NULL	0	NULL	 correction	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Progressive disability can be delayed through a variety of physiatric and orthopedic techniques , including surgical release of lower-extremity contracture , repair of foot and ankle deformity , and correction of scoliosis .
	manualset3
220340	10	420510	7	NULL	NULL	0	NULL	scoliosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Progressive disability can be delayed through a variety of physiatric and orthopedic techniques , including surgical release of lower-extremity contracture , repair of foot and ankle deformity , and correction of scoliosis .
	manualset3
220341	1	420511	7	NULL	NULL	0	NULL	Amastigotes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Amastigotes , sphaeromastigotes , epimastigotes and trypomastigotes of Trypanosoma theileri , Laveran , 1902 have been observed in the nymphs and adults of Hyalomma anatolicum anatolicum ( Koch , 1844 ) .
	manualset3
220342	2	420511	7	NULL	NULL	0	NULL	sphaeromastigotes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Amastigotes , sphaeromastigotes , epimastigotes and trypomastigotes of Trypanosoma theileri , Laveran , 1902 have been observed in the nymphs and adults of Hyalomma anatolicum anatolicum ( Koch , 1844 ) .
	manualset3
220343	3	420511	7	NULL	NULL	0	NULL	epimastigotes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Amastigotes , sphaeromastigotes , epimastigotes and trypomastigotes of Trypanosoma theileri , Laveran , 1902 have been observed in the nymphs and adults of Hyalomma anatolicum anatolicum ( Koch , 1844 ) .
	manualset3
220344	4	420511	7	NULL	NULL	0	NULL	trypomastigotes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Amastigotes , sphaeromastigotes , epimastigotes and trypomastigotes of Trypanosoma theileri , Laveran , 1902 have been observed in the nymphs and adults of Hyalomma anatolicum anatolicum ( Koch , 1844 ) .
	manualset3
220345	5	420511	7	NULL	NULL	0	NULL	Trypanosoma theileri	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Amastigotes , sphaeromastigotes , epimastigotes and trypomastigotes of Trypanosoma theileri , Laveran , 1902 have been observed in the nymphs and adults of Hyalomma anatolicum anatolicum ( Koch , 1844 ) .
	manualset3
220346	6	420511	7	NULL	NULL	0	NULL	Laveran	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Amastigotes , sphaeromastigotes , epimastigotes and trypomastigotes of Trypanosoma theileri , Laveran , 1902 have been observed in the nymphs and adults of Hyalomma anatolicum anatolicum ( Koch , 1844 ) .
	manualset3
220347	7	420511	7	NULL	NULL	0	NULL	1902	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Amastigotes , sphaeromastigotes , epimastigotes and trypomastigotes of Trypanosoma theileri , Laveran , 1902 have been observed in the nymphs and adults of Hyalomma anatolicum anatolicum ( Koch , 1844 ) .
	manualset3
220348	8	420511	7	NULL	NULL	0	NULL	nymphs 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Amastigotes , sphaeromastigotes , epimastigotes and trypomastigotes of Trypanosoma theileri , Laveran , 1902 have been observed in the nymphs and adults of Hyalomma anatolicum anatolicum ( Koch , 1844 ) .
	manualset3
220349	9	420511	7	NULL	NULL	0	NULL	adults	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Amastigotes , sphaeromastigotes , epimastigotes and trypomastigotes of Trypanosoma theileri , Laveran , 1902 have been observed in the nymphs and adults of Hyalomma anatolicum anatolicum ( Koch , 1844 ) .
	manualset3
220350	10	420511	7	NULL	NULL	0	NULL	Hyalomma anatolicum anatolicum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Amastigotes , sphaeromastigotes , epimastigotes and trypomastigotes of Trypanosoma theileri , Laveran , 1902 have been observed in the nymphs and adults of Hyalomma anatolicum anatolicum ( Koch , 1844 ) .
	manualset3
220351	11	420511	7	NULL	NULL	0	NULL	Koch , 1844 	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	Amastigotes , sphaeromastigotes , epimastigotes and trypomastigotes of Trypanosoma theileri , Laveran , 1902 have been observed in the nymphs and adults of Hyalomma anatolicum anatolicum ( Koch , 1844 ) .
	manualset3
220352	1	420512	7	NULL	NULL	0	NULL	Costs	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Costs include direct costs of the drugs used for treatment to JCP from January to February .
	manualset3
220353	2	420512	7	NULL	NULL	0	NULL	direct costs	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Costs include direct costs of the drugs used for treatment to JCP from January to February .
	manualset3
220354	3	420512	7	NULL	NULL	0	NULL	drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Costs include direct costs of the drugs used for treatment to JCP from January to February .
	manualset3
220355	4	420512	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Costs include direct costs of the drugs used for treatment to JCP from January to February .
	manualset3
220356	5	420512	7	NULL	NULL	0	NULL	JCP	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Costs include direct costs of the drugs used for treatment to JCP from January to February .
	manualset3
220357	6	420512	7	NULL	NULL	0	NULL	January	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Costs include direct costs of the drugs used for treatment to JCP from January to February .
	manualset3
220358	7	420512	7	NULL	NULL	0	NULL	 February	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Costs include direct costs of the drugs used for treatment to JCP from January to February .
	manualset3
220359	1	420513	7	NULL	NULL	0	NULL	Lesions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions to the laryngeal cartilages caused by tracheotomy .
	manualset3
220360	2	420513	7	NULL	NULL	0	NULL	laryngeal cartilages	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions to the laryngeal cartilages caused by tracheotomy .
	manualset3
220361	3	420513	7	NULL	NULL	0	NULL	tracheotomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Lesions to the laryngeal cartilages caused by tracheotomy .
	manualset3
220362	1	420514	7	NULL	NULL	0	NULL	In vitro antibacterial activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro antibacterial activity of the peptide deformylase inhibitor BB-83698 .
	manualset3
220363	2	420514	7	NULL	NULL	0	NULL	peptide deformylase inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro antibacterial activity of the peptide deformylase inhibitor BB-83698 .
	manualset3
220364	3	420514	7	NULL	NULL	0	NULL	BB-83698 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In vitro antibacterial activity of the peptide deformylase inhibitor BB-83698 .
	manualset3
220365	1	420515	7	NULL	NULL	NULL	NULL	neuronal protein aggregates	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Notably , neuronal protein aggregates of mutated huntingtin , which is typical HD neuropathology , were not found within the transplanted fetal tissue .
	manualset3
220366	2	420515	7	NULL	NULL	0	NULL	mutated huntingtin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , neuronal protein aggregates of mutated huntingtin , which is typical HD neuropathology , were not found within the transplanted fetal tissue .
	manualset3
220367	3	420515	7	NULL	NULL	NULL	NULL	HD neuropathology	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Notably , neuronal protein aggregates of mutated huntingtin , which is typical HD neuropathology , were not found within the transplanted fetal tissue .
	manualset3
220368	4	420515	7	NULL	NULL	0	NULL	 transplanted fetal tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Notably , neuronal protein aggregates of mutated huntingtin , which is typical HD neuropathology , were not found within the transplanted fetal tissue .
	manualset3
220369	1	420516	7	NULL	NULL	0	NULL	PCBs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	PCBs were determined by liquid gas chromatography on samples taken from workroom air , workroom surfaces and tools , the palms of the hand , and the blood of the workers .
	manualset3
220370	2	420516	7	NULL	NULL	0	NULL	liquid gas chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	PCBs were determined by liquid gas chromatography on samples taken from workroom air , workroom surfaces and tools , the palms of the hand , and the blood of the workers .
	manualset3
220371	3	420516	7	NULL	NULL	0	NULL	samples	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	PCBs were determined by liquid gas chromatography on samples taken from workroom air , workroom surfaces and tools , the palms of the hand , and the blood of the workers .
	manualset3
220372	4	420516	7	NULL	NULL	0	NULL	workroom air	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	PCBs were determined by liquid gas chromatography on samples taken from workroom air , workroom surfaces and tools , the palms of the hand , and the blood of the workers .
	manualset3
220373	5	420516	7	NULL	NULL	0	NULL	workroom surfaces	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	PCBs were determined by liquid gas chromatography on samples taken from workroom air , workroom surfaces and tools , the palms of the hand , and the blood of the workers .
	manualset3
220374	6	420516	7	NULL	NULL	0	NULL	tools	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	PCBs were determined by liquid gas chromatography on samples taken from workroom air , workroom surfaces and tools , the palms of the hand , and the blood of the workers .
	manualset3
220375	7	420516	7	NULL	NULL	0	NULL	palms of the hand	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	PCBs were determined by liquid gas chromatography on samples taken from workroom air , workroom surfaces and tools , the palms of the hand , and the blood of the workers .
	manualset3
220376	8	420516	7	NULL	NULL	0	NULL	blood 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	PCBs were determined by liquid gas chromatography on samples taken from workroom air , workroom surfaces and tools , the palms of the hand , and the blood of the workers .
	manualset3
220377	9	420516	7	NULL	NULL	0	NULL	workers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	PCBs were determined by liquid gas chromatography on samples taken from workroom air , workroom surfaces and tools , the palms of the hand , and the blood of the workers .
	manualset3
220378	1	420517	7	NULL	NULL	0	NULL	compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The others were shown to be known compounds , astrasieversianin XV ( II ) , 7 , 2 ' - dihydroxy-3 ' , 4 ' - dimethoxy-isoflavane-7-O-beta-D-glucoside ( III ) , soyasaponin I , daucosterol and beta-sitosterol .
	manualset3
220379	2	420517	7	NULL	NULL	0	NULL	astrasieversianin XV ( II )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The others were shown to be known compounds , astrasieversianin XV ( II ) , 7 , 2 ' - dihydroxy-3 ' , 4 ' - dimethoxy-isoflavane-7-O-beta-D-glucoside ( III ) , soyasaponin I , daucosterol and beta-sitosterol .
	manualset3
220380	3	420517	7	NULL	NULL	NULL	NULL	7 , 2 ' - dihydroxy-3 ' , 4 ' - dimethoxy-isoflavane-7-O-beta-D-glucoside ( III )	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The others were shown to be known compounds , astrasieversianin XV ( II ) , 7 , 2 ' - dihydroxy-3 ' , 4 ' - dimethoxy-isoflavane-7-O-beta-D-glucoside ( III ) , soyasaponin I , daucosterol and beta-sitosterol .
	manualset3
220381	4	420517	7	NULL	NULL	0	NULL	soyasaponin I	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The others were shown to be known compounds , astrasieversianin XV ( II ) , 7 , 2 ' - dihydroxy-3 ' , 4 ' - dimethoxy-isoflavane-7-O-beta-D-glucoside ( III ) , soyasaponin I , daucosterol and beta-sitosterol .
	manualset3
220382	5	420517	7	NULL	NULL	0	NULL	daucosterol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The others were shown to be known compounds , astrasieversianin XV ( II ) , 7 , 2 ' - dihydroxy-3 ' , 4 ' - dimethoxy-isoflavane-7-O-beta-D-glucoside ( III ) , soyasaponin I , daucosterol and beta-sitosterol .
	manualset3
220383	6	420517	7	NULL	NULL	0	NULL	beta-sitosterol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The others were shown to be known compounds , astrasieversianin XV ( II ) , 7 , 2 ' - dihydroxy-3 ' , 4 ' - dimethoxy-isoflavane-7-O-beta-D-glucoside ( III ) , soyasaponin I , daucosterol and beta-sitosterol .
	manualset3
220384	1	420518	7	NULL	NULL	0	NULL	 alpha chains 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather than protecting alpha chains , the mutant chaperone is partially unfolded but recovers its secondary structure via interaction with alpha-Hb .
	manualset3
220385	2	420518	7	NULL	NULL	0	NULL	mutant chaperone	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather than protecting alpha chains , the mutant chaperone is partially unfolded but recovers its secondary structure via interaction with alpha-Hb .
	manualset3
220386	3	420518	7	NULL	NULL	0	NULL	secondary structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather than protecting alpha chains , the mutant chaperone is partially unfolded but recovers its secondary structure via interaction with alpha-Hb .
	manualset3
220387	4	420518	7	NULL	NULL	0	NULL	 interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather than protecting alpha chains , the mutant chaperone is partially unfolded but recovers its secondary structure via interaction with alpha-Hb .
	manualset3
220388	5	420518	7	NULL	NULL	0	NULL	alpha-Hb	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Rather than protecting alpha chains , the mutant chaperone is partially unfolded but recovers its secondary structure via interaction with alpha-Hb .
	manualset3
220389	1	420519	7	NULL	NULL	0	NULL	Lack 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Lack of effect of melatonin on myometrial electromyographic activity in the pregnant sheep at 138-142 days gestation ( term = 147 days gestation ) .
	manualset3
220390	2	420519	7	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Lack of effect of melatonin on myometrial electromyographic activity in the pregnant sheep at 138-142 days gestation ( term = 147 days gestation ) .
	manualset3
220391	3	420519	7	NULL	NULL	0	NULL	melatonin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lack of effect of melatonin on myometrial electromyographic activity in the pregnant sheep at 138-142 days gestation ( term = 147 days gestation ) .
	manualset3
220392	4	420519	7	NULL	NULL	0	NULL	myometrial electromyographic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lack of effect of melatonin on myometrial electromyographic activity in the pregnant sheep at 138-142 days gestation ( term = 147 days gestation ) .
	manualset3
220393	5	420519	7	NULL	NULL	0	NULL	pregnant sheep	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Lack of effect of melatonin on myometrial electromyographic activity in the pregnant sheep at 138-142 days gestation ( term = 147 days gestation ) .
	manualset3
220394	6	420519	7	NULL	NULL	0	NULL	138-142 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Lack of effect of melatonin on myometrial electromyographic activity in the pregnant sheep at 138-142 days gestation ( term = 147 days gestation ) .
	manualset3
220395	7	420519	7	NULL	NULL	0	NULL	gestation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lack of effect of melatonin on myometrial electromyographic activity in the pregnant sheep at 138-142 days gestation ( term = 147 days gestation ) .
	manualset3
220396	8	420519	7	NULL	NULL	0	NULL	term	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Lack of effect of melatonin on myometrial electromyographic activity in the pregnant sheep at 138-142 days gestation ( term = 147 days gestation ) .
	manualset3
220397	9	420519	7	NULL	NULL	0	NULL	147 days gestation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lack of effect of melatonin on myometrial electromyographic activity in the pregnant sheep at 138-142 days gestation ( term = 147 days gestation ) .
	manualset3
220398	1	420520	7	NULL	NULL	0	NULL	 conservation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Towards the conservation of crucian carp Carassius carassius : understanding the extent and causes of decline within part of its native English range .
	manualset3
220399	2	420520	7	NULL	NULL	0	NULL	crucian carp Carassius carassius	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Towards the conservation of crucian carp Carassius carassius : understanding the extent and causes of decline within part of its native English range .
	manualset3
220400	3	420520	7	NULL	NULL	NULL	NULL	understanding 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Towards the conservation of crucian carp Carassius carassius : understanding the extent and causes of decline within part of its native English range .
	manualset3
220401	4	420520	7	NULL	NULL	0	NULL	causes of decline	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Towards the conservation of crucian carp Carassius carassius : understanding the extent and causes of decline within part of its native English range .
	manualset3
220402	5	420520	7	NULL	NULL	0	NULL	 native English range	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Towards the conservation of crucian carp Carassius carassius : understanding the extent and causes of decline within part of its native English range .
	manualset3
220403	1	420521	7	NULL	NULL	0	NULL	high power input	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , under relatively high power input , the plasma deposition process favored direct surface fluorination .
	manualset3
220404	2	420521	7	NULL	NULL	0	NULL	plasma deposition process 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , under relatively high power input , the plasma deposition process favored direct surface fluorination .
	manualset3
220405	3	420521	7	NULL	NULL	0	NULL	direct surface fluorination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specifically , under relatively high power input , the plasma deposition process favored direct surface fluorination .
	manualset3
220406	1	420522	7	NULL	NULL	0	NULL	Determination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of the time to repeat doses in epidural anesthesia by the change in skin temperature ) .
	manualset3
220407	2	420522	7	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of the time to repeat doses in epidural anesthesia by the change in skin temperature ) .
	manualset3
220408	3	420522	7	NULL	NULL	0	NULL	doses 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of the time to repeat doses in epidural anesthesia by the change in skin temperature ) .
	manualset3
220409	4	420522	7	NULL	NULL	NULL	NULL	epidural anesthesia	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Determination of the time to repeat doses in epidural anesthesia by the change in skin temperature ) .
	manualset3
220410	5	420522	7	NULL	NULL	NULL	NULL	change 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Determination of the time to repeat doses in epidural anesthesia by the change in skin temperature ) .
	manualset3
220411	6	420522	7	NULL	NULL	0	NULL	skin temperature 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of the time to repeat doses in epidural anesthesia by the change in skin temperature ) .
	manualset3
220412	1	420523	7	NULL	NULL	NULL	NULL	method	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The method has been evaluated in plasma from 23 patients on mitotane therapy , revealing DDA concentrations 1-18 times higher than the parent compound .
	manualset3
220413	2	420523	7	NULL	NULL	0	NULL	plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The method has been evaluated in plasma from 23 patients on mitotane therapy , revealing DDA concentrations 1-18 times higher than the parent compound .
	manualset3
220414	3	420523	7	NULL	NULL	0	NULL	23 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The method has been evaluated in plasma from 23 patients on mitotane therapy , revealing DDA concentrations 1-18 times higher than the parent compound .
	manualset3
220415	4	420523	7	NULL	NULL	0	NULL	mitotane therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The method has been evaluated in plasma from 23 patients on mitotane therapy , revealing DDA concentrations 1-18 times higher than the parent compound .
	manualset3
220416	5	420523	7	NULL	NULL	0	NULL	DDA concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method has been evaluated in plasma from 23 patients on mitotane therapy , revealing DDA concentrations 1-18 times higher than the parent compound .
	manualset3
220417	6	420523	7	NULL	NULL	0	NULL	1-18 times 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method has been evaluated in plasma from 23 patients on mitotane therapy , revealing DDA concentrations 1-18 times higher than the parent compound .
	manualset3
220418	7	420523	7	NULL	NULL	0	NULL	 parent compound 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The method has been evaluated in plasma from 23 patients on mitotane therapy , revealing DDA concentrations 1-18 times higher than the parent compound .
	manualset3
220419	1	420524	7	NULL	NULL	0	NULL	Examination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Examination revealed that different N-linker and hinge contacts to the core domain of the partner monomer ( which binds effector molecule ) affect the juxtapositions of the HTH , N-linker , and hinge regions in the DNA binding domain .
	manualset3
220420	2	420524	7	NULL	NULL	0	NULL	different N-linker	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Examination revealed that different N-linker and hinge contacts to the core domain of the partner monomer ( which binds effector molecule ) affect the juxtapositions of the HTH , N-linker , and hinge regions in the DNA binding domain .
	manualset3
220421	3	420524	7	NULL	NULL	0	NULL	hinge contacts	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Examination revealed that different N-linker and hinge contacts to the core domain of the partner monomer ( which binds effector molecule ) affect the juxtapositions of the HTH , N-linker , and hinge regions in the DNA binding domain .
	manualset3
220422	4	420524	7	NULL	NULL	0	NULL	core domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Examination revealed that different N-linker and hinge contacts to the core domain of the partner monomer ( which binds effector molecule ) affect the juxtapositions of the HTH , N-linker , and hinge regions in the DNA binding domain .
	manualset3
220423	5	420524	7	NULL	NULL	0	NULL	partner monomer	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Examination revealed that different N-linker and hinge contacts to the core domain of the partner monomer ( which binds effector molecule ) affect the juxtapositions of the HTH , N-linker , and hinge regions in the DNA binding domain .
	manualset3
220424	6	420524	7	NULL	NULL	0	NULL	effector molecule 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Examination revealed that different N-linker and hinge contacts to the core domain of the partner monomer ( which binds effector molecule ) affect the juxtapositions of the HTH , N-linker , and hinge regions in the DNA binding domain .
	manualset3
220425	7	420524	7	NULL	NULL	0	NULL	 juxtapositions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Examination revealed that different N-linker and hinge contacts to the core domain of the partner monomer ( which binds effector molecule ) affect the juxtapositions of the HTH , N-linker , and hinge regions in the DNA binding domain .
	manualset3
220426	8	420524	7	NULL	NULL	0	NULL	HTH 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Examination revealed that different N-linker and hinge contacts to the core domain of the partner monomer ( which binds effector molecule ) affect the juxtapositions of the HTH , N-linker , and hinge regions in the DNA binding domain .
	manualset3
220427	9	420524	7	NULL	NULL	0	NULL	N-linker	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Examination revealed that different N-linker and hinge contacts to the core domain of the partner monomer ( which binds effector molecule ) affect the juxtapositions of the HTH , N-linker , and hinge regions in the DNA binding domain .
	manualset3
220428	10	420524	7	NULL	NULL	0	NULL	hinge regions	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Examination revealed that different N-linker and hinge contacts to the core domain of the partner monomer ( which binds effector molecule ) affect the juxtapositions of the HTH , N-linker , and hinge regions in the DNA binding domain .
	manualset3
220429	11	420524	7	NULL	NULL	0	NULL	DNA binding domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Examination revealed that different N-linker and hinge contacts to the core domain of the partner monomer ( which binds effector molecule ) affect the juxtapositions of the HTH , N-linker , and hinge regions in the DNA binding domain .
	manualset3
220430	1	420525	7	NULL	NULL	0	NULL	AtT-20 neuroendocrine cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , AtT-20 neuroendocrine cells were transfected with wild-type and mutated TH genes because these cells were earlier shown to be capable of fully converting L-3 , 4 - dihydroxyphenylalanine into DA , whereby the catalytic activity of TH would be expected to be inhibited by the end product DA accumulating in the cells .
	manualset3
220431	2	420525	7	NULL	NULL	0	NULL	 wild-type genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , AtT-20 neuroendocrine cells were transfected with wild-type and mutated TH genes because these cells were earlier shown to be capable of fully converting L-3 , 4 - dihydroxyphenylalanine into DA , whereby the catalytic activity of TH would be expected to be inhibited by the end product DA accumulating in the cells .
	manualset3
220432	3	420525	7	NULL	NULL	0	NULL	mutated TH genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , AtT-20 neuroendocrine cells were transfected with wild-type and mutated TH genes because these cells were earlier shown to be capable of fully converting L-3 , 4 - dihydroxyphenylalanine into DA , whereby the catalytic activity of TH would be expected to be inhibited by the end product DA accumulating in the cells .
	manualset3
220433	4	420525	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , AtT-20 neuroendocrine cells were transfected with wild-type and mutated TH genes because these cells were earlier shown to be capable of fully converting L-3 , 4 - dihydroxyphenylalanine into DA , whereby the catalytic activity of TH would be expected to be inhibited by the end product DA accumulating in the cells .
	manualset3
220434	5	420525	7	NULL	NULL	0	NULL	L-3 , 4 - dihydroxyphenylalanine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , AtT-20 neuroendocrine cells were transfected with wild-type and mutated TH genes because these cells were earlier shown to be capable of fully converting L-3 , 4 - dihydroxyphenylalanine into DA , whereby the catalytic activity of TH would be expected to be inhibited by the end product DA accumulating in the cells .
	manualset3
220435	6	420525	7	NULL	NULL	0	NULL	DA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , AtT-20 neuroendocrine cells were transfected with wild-type and mutated TH genes because these cells were earlier shown to be capable of fully converting L-3 , 4 - dihydroxyphenylalanine into DA , whereby the catalytic activity of TH would be expected to be inhibited by the end product DA accumulating in the cells .
	manualset3
220436	7	420525	7	NULL	NULL	0	NULL	 catalytic activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , AtT-20 neuroendocrine cells were transfected with wild-type and mutated TH genes because these cells were earlier shown to be capable of fully converting L-3 , 4 - dihydroxyphenylalanine into DA , whereby the catalytic activity of TH would be expected to be inhibited by the end product DA accumulating in the cells .
	manualset3
220437	8	420525	7	NULL	NULL	NULL	NULL	TH	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Next , AtT-20 neuroendocrine cells were transfected with wild-type and mutated TH genes because these cells were earlier shown to be capable of fully converting L-3 , 4 - dihydroxyphenylalanine into DA , whereby the catalytic activity of TH would be expected to be inhibited by the end product DA accumulating in the cells .
	manualset3
220438	9	420525	7	NULL	NULL	0	NULL	end product DA 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , AtT-20 neuroendocrine cells were transfected with wild-type and mutated TH genes because these cells were earlier shown to be capable of fully converting L-3 , 4 - dihydroxyphenylalanine into DA , whereby the catalytic activity of TH would be expected to be inhibited by the end product DA accumulating in the cells .
	manualset3
220439	10	420525	7	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Next , AtT-20 neuroendocrine cells were transfected with wild-type and mutated TH genes because these cells were earlier shown to be capable of fully converting L-3 , 4 - dihydroxyphenylalanine into DA , whereby the catalytic activity of TH would be expected to be inhibited by the end product DA accumulating in the cells .
	manualset3
220440	1	420526	7	NULL	NULL	0	NULL	method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This method has advantages in its ( 1 ) objectivity of the judgement because of the clear difference of the dry up patterns between positive reaction and negative , ( 2 ) shortness of the handling time ( results can be obtained within 2 hr from sampling ) , ( 3 ) requirement of little amount of sample and of Limulus lysate ( a fifth volume of sample and a tenth volume of lysate are needed compared with the conventional method ) and ( 4 ) sensitivity ( 0.1 or 0.5 ng/ml of lipopolysaccharide ( LPS ) ) .
	manualset3
220441	2	420526	7	NULL	NULL	0	NULL	objectivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This method has advantages in its ( 1 ) objectivity of the judgement because of the clear difference of the dry up patterns between positive reaction and negative , ( 2 ) shortness of the handling time ( results can be obtained within 2 hr from sampling ) , ( 3 ) requirement of little amount of sample and of Limulus lysate ( a fifth volume of sample and a tenth volume of lysate are needed compared with the conventional method ) and ( 4 ) sensitivity ( 0.1 or 0.5 ng/ml of lipopolysaccharide ( LPS ) ) .
	manualset3
220442	3	420526	7	NULL	NULL	0	NULL	 judgement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This method has advantages in its ( 1 ) objectivity of the judgement because of the clear difference of the dry up patterns between positive reaction and negative , ( 2 ) shortness of the handling time ( results can be obtained within 2 hr from sampling ) , ( 3 ) requirement of little amount of sample and of Limulus lysate ( a fifth volume of sample and a tenth volume of lysate are needed compared with the conventional method ) and ( 4 ) sensitivity ( 0.1 or 0.5 ng/ml of lipopolysaccharide ( LPS ) ) .
	manualset3
220443	4	420526	7	NULL	NULL	0	NULL	clear difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	This method has advantages in its ( 1 ) objectivity of the judgement because of the clear difference of the dry up patterns between positive reaction and negative , ( 2 ) shortness of the handling time ( results can be obtained within 2 hr from sampling ) , ( 3 ) requirement of little amount of sample and of Limulus lysate ( a fifth volume of sample and a tenth volume of lysate are needed compared with the conventional method ) and ( 4 ) sensitivity ( 0.1 or 0.5 ng/ml of lipopolysaccharide ( LPS ) ) .
	manualset3
220444	5	420526	7	NULL	NULL	0	NULL	 dry up patterns	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This method has advantages in its ( 1 ) objectivity of the judgement because of the clear difference of the dry up patterns between positive reaction and negative , ( 2 ) shortness of the handling time ( results can be obtained within 2 hr from sampling ) , ( 3 ) requirement of little amount of sample and of Limulus lysate ( a fifth volume of sample and a tenth volume of lysate are needed compared with the conventional method ) and ( 4 ) sensitivity ( 0.1 or 0.5 ng/ml of lipopolysaccharide ( LPS ) ) .
	manualset3
220445	6	420526	7	NULL	NULL	0	NULL	positive reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This method has advantages in its ( 1 ) objectivity of the judgement because of the clear difference of the dry up patterns between positive reaction and negative , ( 2 ) shortness of the handling time ( results can be obtained within 2 hr from sampling ) , ( 3 ) requirement of little amount of sample and of Limulus lysate ( a fifth volume of sample and a tenth volume of lysate are needed compared with the conventional method ) and ( 4 ) sensitivity ( 0.1 or 0.5 ng/ml of lipopolysaccharide ( LPS ) ) .
	manualset3
220446	7	420526	7	NULL	NULL	0	NULL	negative reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This method has advantages in its ( 1 ) objectivity of the judgement because of the clear difference of the dry up patterns between positive reaction and negative , ( 2 ) shortness of the handling time ( results can be obtained within 2 hr from sampling ) , ( 3 ) requirement of little amount of sample and of Limulus lysate ( a fifth volume of sample and a tenth volume of lysate are needed compared with the conventional method ) and ( 4 ) sensitivity ( 0.1 or 0.5 ng/ml of lipopolysaccharide ( LPS ) ) .
	manualset3
220447	8	420526	7	NULL	NULL	0	NULL	shortness	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	This method has advantages in its ( 1 ) objectivity of the judgement because of the clear difference of the dry up patterns between positive reaction and negative , ( 2 ) shortness of the handling time ( results can be obtained within 2 hr from sampling ) , ( 3 ) requirement of little amount of sample and of Limulus lysate ( a fifth volume of sample and a tenth volume of lysate are needed compared with the conventional method ) and ( 4 ) sensitivity ( 0.1 or 0.5 ng/ml of lipopolysaccharide ( LPS ) ) .
	manualset3
220448	9	420526	7	NULL	NULL	0	NULL	handling time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	This method has advantages in its ( 1 ) objectivity of the judgement because of the clear difference of the dry up patterns between positive reaction and negative , ( 2 ) shortness of the handling time ( results can be obtained within 2 hr from sampling ) , ( 3 ) requirement of little amount of sample and of Limulus lysate ( a fifth volume of sample and a tenth volume of lysate are needed compared with the conventional method ) and ( 4 ) sensitivity ( 0.1 or 0.5 ng/ml of lipopolysaccharide ( LPS ) ) .
	manualset3
220449	10	420526	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This method has advantages in its ( 1 ) objectivity of the judgement because of the clear difference of the dry up patterns between positive reaction and negative , ( 2 ) shortness of the handling time ( results can be obtained within 2 hr from sampling ) , ( 3 ) requirement of little amount of sample and of Limulus lysate ( a fifth volume of sample and a tenth volume of lysate are needed compared with the conventional method ) and ( 4 ) sensitivity ( 0.1 or 0.5 ng/ml of lipopolysaccharide ( LPS ) ) .
	manualset3
220450	11	420526	7	NULL	NULL	0	NULL	2 hr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	This method has advantages in its ( 1 ) objectivity of the judgement because of the clear difference of the dry up patterns between positive reaction and negative , ( 2 ) shortness of the handling time ( results can be obtained within 2 hr from sampling ) , ( 3 ) requirement of little amount of sample and of Limulus lysate ( a fifth volume of sample and a tenth volume of lysate are needed compared with the conventional method ) and ( 4 ) sensitivity ( 0.1 or 0.5 ng/ml of lipopolysaccharide ( LPS ) ) .
	manualset3
220451	12	420526	7	NULL	NULL	0	NULL	sampling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This method has advantages in its ( 1 ) objectivity of the judgement because of the clear difference of the dry up patterns between positive reaction and negative , ( 2 ) shortness of the handling time ( results can be obtained within 2 hr from sampling ) , ( 3 ) requirement of little amount of sample and of Limulus lysate ( a fifth volume of sample and a tenth volume of lysate are needed compared with the conventional method ) and ( 4 ) sensitivity ( 0.1 or 0.5 ng/ml of lipopolysaccharide ( LPS ) ) .
	manualset3
220452	13	420526	7	NULL	NULL	0	NULL	requirement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This method has advantages in its ( 1 ) objectivity of the judgement because of the clear difference of the dry up patterns between positive reaction and negative , ( 2 ) shortness of the handling time ( results can be obtained within 2 hr from sampling ) , ( 3 ) requirement of little amount of sample and of Limulus lysate ( a fifth volume of sample and a tenth volume of lysate are needed compared with the conventional method ) and ( 4 ) sensitivity ( 0.1 or 0.5 ng/ml of lipopolysaccharide ( LPS ) ) .
	manualset3
220453	14	420526	7	NULL	NULL	0	NULL	 little amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This method has advantages in its ( 1 ) objectivity of the judgement because of the clear difference of the dry up patterns between positive reaction and negative , ( 2 ) shortness of the handling time ( results can be obtained within 2 hr from sampling ) , ( 3 ) requirement of little amount of sample and of Limulus lysate ( a fifth volume of sample and a tenth volume of lysate are needed compared with the conventional method ) and ( 4 ) sensitivity ( 0.1 or 0.5 ng/ml of lipopolysaccharide ( LPS ) ) .
	manualset3
220454	15	420526	7	NULL	NULL	0	NULL	sample	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	This method has advantages in its ( 1 ) objectivity of the judgement because of the clear difference of the dry up patterns between positive reaction and negative , ( 2 ) shortness of the handling time ( results can be obtained within 2 hr from sampling ) , ( 3 ) requirement of little amount of sample and of Limulus lysate ( a fifth volume of sample and a tenth volume of lysate are needed compared with the conventional method ) and ( 4 ) sensitivity ( 0.1 or 0.5 ng/ml of lipopolysaccharide ( LPS ) ) .
	manualset3
220455	16	420526	7	NULL	NULL	0	NULL	Limulus lysate	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This method has advantages in its ( 1 ) objectivity of the judgement because of the clear difference of the dry up patterns between positive reaction and negative , ( 2 ) shortness of the handling time ( results can be obtained within 2 hr from sampling ) , ( 3 ) requirement of little amount of sample and of Limulus lysate ( a fifth volume of sample and a tenth volume of lysate are needed compared with the conventional method ) and ( 4 ) sensitivity ( 0.1 or 0.5 ng/ml of lipopolysaccharide ( LPS ) ) .
	manualset3
220456	17	420526	7	NULL	NULL	0	NULL	fifth volume	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This method has advantages in its ( 1 ) objectivity of the judgement because of the clear difference of the dry up patterns between positive reaction and negative , ( 2 ) shortness of the handling time ( results can be obtained within 2 hr from sampling ) , ( 3 ) requirement of little amount of sample and of Limulus lysate ( a fifth volume of sample and a tenth volume of lysate are needed compared with the conventional method ) and ( 4 ) sensitivity ( 0.1 or 0.5 ng/ml of lipopolysaccharide ( LPS ) ) .
	manualset3
220457	18	420526	7	NULL	NULL	0	NULL	sample 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	This method has advantages in its ( 1 ) objectivity of the judgement because of the clear difference of the dry up patterns between positive reaction and negative , ( 2 ) shortness of the handling time ( results can be obtained within 2 hr from sampling ) , ( 3 ) requirement of little amount of sample and of Limulus lysate ( a fifth volume of sample and a tenth volume of lysate are needed compared with the conventional method ) and ( 4 ) sensitivity ( 0.1 or 0.5 ng/ml of lipopolysaccharide ( LPS ) ) .
	manualset3
220458	19	420526	7	NULL	NULL	0	NULL	tenth volume	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This method has advantages in its ( 1 ) objectivity of the judgement because of the clear difference of the dry up patterns between positive reaction and negative , ( 2 ) shortness of the handling time ( results can be obtained within 2 hr from sampling ) , ( 3 ) requirement of little amount of sample and of Limulus lysate ( a fifth volume of sample and a tenth volume of lysate are needed compared with the conventional method ) and ( 4 ) sensitivity ( 0.1 or 0.5 ng/ml of lipopolysaccharide ( LPS ) ) .
	manualset3
220459	20	420526	7	NULL	NULL	0	NULL	 lysate 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This method has advantages in its ( 1 ) objectivity of the judgement because of the clear difference of the dry up patterns between positive reaction and negative , ( 2 ) shortness of the handling time ( results can be obtained within 2 hr from sampling ) , ( 3 ) requirement of little amount of sample and of Limulus lysate ( a fifth volume of sample and a tenth volume of lysate are needed compared with the conventional method ) and ( 4 ) sensitivity ( 0.1 or 0.5 ng/ml of lipopolysaccharide ( LPS ) ) .
	manualset3
220460	21	420526	7	NULL	NULL	0	NULL	conventional method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This method has advantages in its ( 1 ) objectivity of the judgement because of the clear difference of the dry up patterns between positive reaction and negative , ( 2 ) shortness of the handling time ( results can be obtained within 2 hr from sampling ) , ( 3 ) requirement of little amount of sample and of Limulus lysate ( a fifth volume of sample and a tenth volume of lysate are needed compared with the conventional method ) and ( 4 ) sensitivity ( 0.1 or 0.5 ng/ml of lipopolysaccharide ( LPS ) ) .
	manualset3
220461	22	420526	7	NULL	NULL	0	NULL	 sensitivity 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This method has advantages in its ( 1 ) objectivity of the judgement because of the clear difference of the dry up patterns between positive reaction and negative , ( 2 ) shortness of the handling time ( results can be obtained within 2 hr from sampling ) , ( 3 ) requirement of little amount of sample and of Limulus lysate ( a fifth volume of sample and a tenth volume of lysate are needed compared with the conventional method ) and ( 4 ) sensitivity ( 0.1 or 0.5 ng/ml of lipopolysaccharide ( LPS ) ) .
	manualset3
220462	23	420526	7	NULL	NULL	0	NULL	0.1 or 0.5 ng/ml	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This method has advantages in its ( 1 ) objectivity of the judgement because of the clear difference of the dry up patterns between positive reaction and negative , ( 2 ) shortness of the handling time ( results can be obtained within 2 hr from sampling ) , ( 3 ) requirement of little amount of sample and of Limulus lysate ( a fifth volume of sample and a tenth volume of lysate are needed compared with the conventional method ) and ( 4 ) sensitivity ( 0.1 or 0.5 ng/ml of lipopolysaccharide ( LPS ) ) .
	manualset3
220463	24	420526	7	NULL	NULL	0	NULL	lipopolysaccharide ( LPS ) )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This method has advantages in its ( 1 ) objectivity of the judgement because of the clear difference of the dry up patterns between positive reaction and negative , ( 2 ) shortness of the handling time ( results can be obtained within 2 hr from sampling ) , ( 3 ) requirement of little amount of sample and of Limulus lysate ( a fifth volume of sample and a tenth volume of lysate are needed compared with the conventional method ) and ( 4 ) sensitivity ( 0.1 or 0.5 ng/ml of lipopolysaccharide ( LPS ) ) .
	manualset3
220464	1	420527	7	NULL	NULL	0	NULL	Current smokers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Current smokers had a shorter time to onset of claudication pain ( p = 0.023 ) and shorter maximal claudication pain times ( p = 0.029 ) than former or never smokers ( p = 0.023 ) .
	manualset3
220465	2	420527	7	NULL	NULL	0	NULL	shorter time	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Current smokers had a shorter time to onset of claudication pain ( p = 0.023 ) and shorter maximal claudication pain times ( p = 0.029 ) than former or never smokers ( p = 0.023 ) .
	manualset3
220466	3	420527	7	NULL	NULL	NULL	NULL	onset of claudication pain	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current smokers had a shorter time to onset of claudication pain ( p = 0.023 ) and shorter maximal claudication pain times ( p = 0.029 ) than former or never smokers ( p = 0.023 ) .
	manualset3
220467	4	420527	7	NULL	NULL	0	NULL	 p = 0.023	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Current smokers had a shorter time to onset of claudication pain ( p = 0.023 ) and shorter maximal claudication pain times ( p = 0.029 ) than former or never smokers ( p = 0.023 ) .
	manualset3
220468	5	420527	7	NULL	NULL	0	NULL	shorter maximal claudication pain times	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Current smokers had a shorter time to onset of claudication pain ( p = 0.023 ) and shorter maximal claudication pain times ( p = 0.029 ) than former or never smokers ( p = 0.023 ) .
	manualset3
220469	6	420527	7	NULL	NULL	0	NULL	 p = 0.029	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Current smokers had a shorter time to onset of claudication pain ( p = 0.023 ) and shorter maximal claudication pain times ( p = 0.029 ) than former or never smokers ( p = 0.023 ) .
	manualset3
220470	7	420527	7	NULL	NULL	0	NULL	 smokers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Current smokers had a shorter time to onset of claudication pain ( p = 0.023 ) and shorter maximal claudication pain times ( p = 0.029 ) than former or never smokers ( p = 0.023 ) .
	manualset3
220471	8	420527	7	NULL	NULL	0	NULL	p = 0.023 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Current smokers had a shorter time to onset of claudication pain ( p = 0.023 ) and shorter maximal claudication pain times ( p = 0.029 ) than former or never smokers ( p = 0.023 ) .
	manualset3
220472	1	420528	7	NULL	NULL	0	NULL	Details 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Details regarding claims of rubella occurred in Lombardia ( Italy ) have been collected by the AA. , in force at the Regional Health Services .
	manualset3
220473	2	420528	7	NULL	NULL	0	NULL	claims	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Details regarding claims of rubella occurred in Lombardia ( Italy ) have been collected by the AA. , in force at the Regional Health Services .
	manualset3
220474	3	420528	7	NULL	NULL	0	NULL	 rubella	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Details regarding claims of rubella occurred in Lombardia ( Italy ) have been collected by the AA. , in force at the Regional Health Services .
	manualset3
220475	4	420528	7	NULL	NULL	0	NULL	Lombardia ( Italy )	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Details regarding claims of rubella occurred in Lombardia ( Italy ) have been collected by the AA. , in force at the Regional Health Services .
	manualset3
220476	5	420528	7	NULL	NULL	0	NULL	AA	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Details regarding claims of rubella occurred in Lombardia ( Italy ) have been collected by the AA. , in force at the Regional Health Services .
	manualset3
220477	6	420528	7	NULL	NULL	0	NULL	force 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Details regarding claims of rubella occurred in Lombardia ( Italy ) have been collected by the AA. , in force at the Regional Health Services .
	manualset3
220478	7	420528	7	NULL	NULL	0	NULL	Regional Health Services	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Details regarding claims of rubella occurred in Lombardia ( Italy ) have been collected by the AA. , in force at the Regional Health Services .
	manualset3
220479	1	420529	7	NULL	NULL	0	NULL	Ambroise Tardieu	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Ambroise Tardieu : the man and his work on child maltreatment a century before Kempe .
	manualset3
220480	2	420529	7	NULL	NULL	0	NULL	 man	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Ambroise Tardieu : the man and his work on child maltreatment a century before Kempe .
	manualset3
220481	3	420529	7	NULL	NULL	0	NULL	work	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ambroise Tardieu : the man and his work on child maltreatment a century before Kempe .
	manualset3
220482	4	420529	7	NULL	NULL	0	NULL	child maltreatment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ambroise Tardieu : the man and his work on child maltreatment a century before Kempe .
	manualset3
220483	5	420529	7	NULL	NULL	0	NULL	century 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Ambroise Tardieu : the man and his work on child maltreatment a century before Kempe .
	manualset3
220484	6	420529	7	NULL	NULL	0	NULL	Kempe 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Ambroise Tardieu : the man and his work on child maltreatment a century before Kempe .
	manualset3
220485	1	420530	7	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of sulfhydryl active agents on insulin binding to the erythrocyte insulin receptor .
	manualset3
220486	2	420530	7	NULL	NULL	0	NULL	sulfhydryl active agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of sulfhydryl active agents on insulin binding to the erythrocyte insulin receptor .
	manualset3
220487	3	420530	7	NULL	NULL	0	NULL	insulin binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of sulfhydryl active agents on insulin binding to the erythrocyte insulin receptor .
	manualset3
220488	4	420530	7	NULL	NULL	0	NULL	erythrocyte insulin receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of sulfhydryl active agents on insulin binding to the erythrocyte insulin receptor .
	manualset3
220508	1	420531	7	NULL	NULL	0	NULL	AcrB	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These are AcrB , TolC , and AcrA , respectively , in Escherichia coli .
	manualset3
220509	2	420531	7	NULL	NULL	0	NULL	TolC	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These are AcrB , TolC , and AcrA , respectively , in Escherichia coli .
	manualset3
220510	3	420531	7	NULL	NULL	0	NULL	AcrA	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These are AcrB , TolC , and AcrA , respectively , in Escherichia coli .
	manualset3
220511	4	420531	7	NULL	NULL	0	NULL	Escherichia coli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These are AcrB , TolC , and AcrA , respectively , in Escherichia coli .
	manualset3
220517	1	420533	7	NULL	NULL	0	NULL	long intervals	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when discriminating long intervals , CD patients also showed a precision deficit , which points to impaired sustained attention and/or decision processes .
	manualset3
220518	2	420533	7	NULL	NULL	0	NULL	CD patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when discriminating long intervals , CD patients also showed a precision deficit , which points to impaired sustained attention and/or decision processes .
	manualset3
220519	3	420533	7	NULL	NULL	0	NULL	precision deficit	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when discriminating long intervals , CD patients also showed a precision deficit , which points to impaired sustained attention and/or decision processes .
	manualset3
220520	4	420533	7	NULL	NULL	0	NULL	 impaired sustained attention	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when discriminating long intervals , CD patients also showed a precision deficit , which points to impaired sustained attention and/or decision processes .
	manualset3
220521	5	420533	7	NULL	NULL	0	NULL	decision processes 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , when discriminating long intervals , CD patients also showed a precision deficit , which points to impaired sustained attention and/or decision processes .
	manualset3
220522	1	420534	7	NULL	NULL	NULL	NULL	borohydride/GC method	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A simple borohydride/GC method was developed for phenotyping sparteine oxidation in man .
	manualset3
220523	2	420534	7	NULL	NULL	0	NULL	phenotyping	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple borohydride/GC method was developed for phenotyping sparteine oxidation in man .
	manualset3
220524	3	420534	7	NULL	NULL	0	NULL	sparteine oxidation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple borohydride/GC method was developed for phenotyping sparteine oxidation in man .
	manualset3
220525	4	420534	7	NULL	NULL	0	NULL	man	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A simple borohydride/GC method was developed for phenotyping sparteine oxidation in man .
	manualset3
220526	1	420535	7	NULL	NULL	0	NULL	 regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of NGF synthesis , and the recruitment of white blood cells , macrophages in particular , from blood into the damaged nerve tissue , are two such mechanisms .
	manualset3
220527	2	420535	7	NULL	NULL	0	NULL	NGF synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of NGF synthesis , and the recruitment of white blood cells , macrophages in particular , from blood into the damaged nerve tissue , are two such mechanisms .
	manualset3
220528	3	420535	7	NULL	NULL	NULL	NULL	recruitment	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The regulation of NGF synthesis , and the recruitment of white blood cells , macrophages in particular , from blood into the damaged nerve tissue , are two such mechanisms .
	manualset3
220529	4	420535	7	NULL	NULL	0	NULL	white blood cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of NGF synthesis , and the recruitment of white blood cells , macrophages in particular , from blood into the damaged nerve tissue , are two such mechanisms .
	manualset3
220530	5	420535	7	NULL	NULL	0	NULL	macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of NGF synthesis , and the recruitment of white blood cells , macrophages in particular , from blood into the damaged nerve tissue , are two such mechanisms .
	manualset3
220531	6	420535	7	NULL	NULL	0	NULL	blood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of NGF synthesis , and the recruitment of white blood cells , macrophages in particular , from blood into the damaged nerve tissue , are two such mechanisms .
	manualset3
220532	7	420535	7	NULL	NULL	0	NULL	damaged nerve tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of NGF synthesis , and the recruitment of white blood cells , macrophages in particular , from blood into the damaged nerve tissue , are two such mechanisms .
	manualset3
220533	8	420535	7	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of NGF synthesis , and the recruitment of white blood cells , macrophages in particular , from blood into the damaged nerve tissue , are two such mechanisms .
	manualset3
220534	9	420535	7	NULL	NULL	0	NULL	mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The regulation of NGF synthesis , and the recruitment of white blood cells , macrophages in particular , from blood into the damaged nerve tissue , are two such mechanisms .
	manualset3
220535	1	420536	7	NULL	NULL	0	NULL	application 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of chemically activated 4-META resin using the brush-dip technique was an effective surface preparation for the bonding of a gingival shade composite resin to a denture base resin .
	manualset3
220536	2	420536	7	NULL	NULL	0	NULL	4-META resin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of chemically activated 4-META resin using the brush-dip technique was an effective surface preparation for the bonding of a gingival shade composite resin to a denture base resin .
	manualset3
220537	3	420536	7	NULL	NULL	0	NULL	brush-dip technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of chemically activated 4-META resin using the brush-dip technique was an effective surface preparation for the bonding of a gingival shade composite resin to a denture base resin .
	manualset3
220538	4	420536	7	NULL	NULL	0	NULL	effective surface preparation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of chemically activated 4-META resin using the brush-dip technique was an effective surface preparation for the bonding of a gingival shade composite resin to a denture base resin .
	manualset3
220539	5	420536	7	NULL	NULL	0	NULL	bonding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of chemically activated 4-META resin using the brush-dip technique was an effective surface preparation for the bonding of a gingival shade composite resin to a denture base resin .
	manualset3
220540	6	420536	7	NULL	NULL	0	NULL	gingival shade composite resin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of chemically activated 4-META resin using the brush-dip technique was an effective surface preparation for the bonding of a gingival shade composite resin to a denture base resin .
	manualset3
220541	7	420536	7	NULL	NULL	0	NULL	base resin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The application of chemically activated 4-META resin using the brush-dip technique was an effective surface preparation for the bonding of a gingival shade composite resin to a denture base resin .
	manualset3
220542	1	420537	7	NULL	NULL	0	NULL	Ambulatory blood pressure measurement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ambulatory blood pressure measurement and antihypertensive therapy .
	manualset3
220543	2	420537	7	NULL	NULL	0	NULL	antihypertensive therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ambulatory blood pressure measurement and antihypertensive therapy .
	manualset3
220544	1	420538	7	NULL	NULL	0	NULL	Effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of buffer , pH , ionic strength and temperatures on lactate dehydrogenase isozymes .
	manualset3
220545	2	420538	7	NULL	NULL	0	NULL	buffer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of buffer , pH , ionic strength and temperatures on lactate dehydrogenase isozymes .
	manualset3
220546	3	420538	7	NULL	NULL	0	NULL	pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of buffer , pH , ionic strength and temperatures on lactate dehydrogenase isozymes .
	manualset3
220547	4	420538	7	NULL	NULL	0	NULL	ionic strength	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of buffer , pH , ionic strength and temperatures on lactate dehydrogenase isozymes .
	manualset3
220548	5	420538	7	NULL	NULL	0	NULL	temperatures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of buffer , pH , ionic strength and temperatures on lactate dehydrogenase isozymes .
	manualset3
220549	6	420538	7	NULL	NULL	0	NULL	lactate dehydrogenase isozymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of buffer , pH , ionic strength and temperatures on lactate dehydrogenase isozymes .
	manualset3
220550	1	420539	7	NULL	NULL	0	NULL	Metastases 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Metastases from malignant tumors beyond the knee and elbow are uncommon and represent only 1 to 2 % of all bone metastases .
	manualset3
220551	2	420539	7	NULL	NULL	0	NULL	malignant tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Metastases from malignant tumors beyond the knee and elbow are uncommon and represent only 1 to 2 % of all bone metastases .
	manualset3
220552	3	420539	7	NULL	NULL	0	NULL	knee	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Metastases from malignant tumors beyond the knee and elbow are uncommon and represent only 1 to 2 % of all bone metastases .
	manualset3
220553	4	420539	7	NULL	NULL	0	NULL	elbow	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Metastases from malignant tumors beyond the knee and elbow are uncommon and represent only 1 to 2 % of all bone metastases .
	manualset3
220554	5	420539	7	NULL	NULL	0	NULL	1 to 2 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Metastases from malignant tumors beyond the knee and elbow are uncommon and represent only 1 to 2 % of all bone metastases .
	manualset3
220555	6	420539	7	NULL	NULL	0	NULL	bone metastases	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Metastases from malignant tumors beyond the knee and elbow are uncommon and represent only 1 to 2 % of all bone metastases .
	manualset3
220556	1	420540	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	From the above results , we suggest that MotX and MotY of the T ring are involved in the incorporation and/or stabilization of the PomA/PomB complex in the motor .
	manualset3
220557	2	420540	7	NULL	NULL	0	NULL	MotX 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	From the above results , we suggest that MotX and MotY of the T ring are involved in the incorporation and/or stabilization of the PomA/PomB complex in the motor .
	manualset3
220558	3	420540	7	NULL	NULL	0	NULL	MotY	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	From the above results , we suggest that MotX and MotY of the T ring are involved in the incorporation and/or stabilization of the PomA/PomB complex in the motor .
	manualset3
220559	4	420540	7	NULL	NULL	0	NULL	 T ring 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	From the above results , we suggest that MotX and MotY of the T ring are involved in the incorporation and/or stabilization of the PomA/PomB complex in the motor .
	manualset3
220560	5	420540	7	NULL	NULL	0	NULL	incorporation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	From the above results , we suggest that MotX and MotY of the T ring are involved in the incorporation and/or stabilization of the PomA/PomB complex in the motor .
	manualset3
220561	6	420540	7	NULL	NULL	0	NULL	stabilization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	From the above results , we suggest that MotX and MotY of the T ring are involved in the incorporation and/or stabilization of the PomA/PomB complex in the motor .
	manualset3
220562	7	420540	7	NULL	NULL	0	NULL	PomA/PomB complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	From the above results , we suggest that MotX and MotY of the T ring are involved in the incorporation and/or stabilization of the PomA/PomB complex in the motor .
	manualset3
220563	8	420540	7	NULL	NULL	0	NULL	motor	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	From the above results , we suggest that MotX and MotY of the T ring are involved in the incorporation and/or stabilization of the PomA/PomB complex in the motor .
	manualset3
220564	1	420541	7	NULL	NULL	0	NULL	Recombinant adeno-associated viruses ( rAAV )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant adeno-associated viruses ( rAAV ) are attractive tools for gene therapy .
	manualset3
220565	2	420541	7	NULL	NULL	0	NULL	tools	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant adeno-associated viruses ( rAAV ) are attractive tools for gene therapy .
	manualset3
220566	3	420541	7	NULL	NULL	0	NULL	gene therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant adeno-associated viruses ( rAAV ) are attractive tools for gene therapy .
	manualset3
220567	1	420542	7	NULL	NULL	0	NULL	GRFT	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We show that GRFT , unlike CV-N , binds the surface of human epithelial and peripheral blood mononuclear cells ( PBMC ) through an exclusively oligosaccharide-dependent interaction .
	manualset3
220568	2	420542	7	NULL	NULL	0	NULL	CV-N	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We show that GRFT , unlike CV-N , binds the surface of human epithelial and peripheral blood mononuclear cells ( PBMC ) through an exclusively oligosaccharide-dependent interaction .
	manualset3
220569	3	420542	7	NULL	NULL	0	NULL	surface	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We show that GRFT , unlike CV-N , binds the surface of human epithelial and peripheral blood mononuclear cells ( PBMC ) through an exclusively oligosaccharide-dependent interaction .
	manualset3
220570	4	420542	7	NULL	NULL	0	NULL	human epithelial and peripheral blood mononuclear cells ( PBMC ) 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We show that GRFT , unlike CV-N , binds the surface of human epithelial and peripheral blood mononuclear cells ( PBMC ) through an exclusively oligosaccharide-dependent interaction .
	manualset3
220571	5	420542	7	NULL	NULL	0	NULL	oligosaccharide-dependent interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We show that GRFT , unlike CV-N , binds the surface of human epithelial and peripheral blood mononuclear cells ( PBMC ) through an exclusively oligosaccharide-dependent interaction .
	manualset3
220572	1	420543	7	NULL	NULL	0	NULL	Effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Effect of aminomethylcyclohexane carboxylic acid on the behavior of erythrocytes injected intraperitoneally .
	manualset3
220573	2	420543	7	NULL	NULL	0	NULL	aminomethylcyclohexane carboxylic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Effect of aminomethylcyclohexane carboxylic acid on the behavior of erythrocytes injected intraperitoneally .
	manualset3
220574	3	420543	7	NULL	NULL	NULL	NULL	 behavior	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of aminomethylcyclohexane carboxylic acid on the behavior of erythrocytes injected intraperitoneally .
	manualset3
220575	4	420543	7	NULL	NULL	0	NULL	 erythrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Effect of aminomethylcyclohexane carboxylic acid on the behavior of erythrocytes injected intraperitoneally .
	manualset3
220576	1	420544	7	NULL	NULL	0	NULL	determination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of serum choline concentrations was carried out by tandem-mass spectroscopy .
	manualset3
220577	2	420544	7	NULL	NULL	0	NULL	serum choline concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of serum choline concentrations was carried out by tandem-mass spectroscopy .
	manualset3
220578	3	420544	7	NULL	NULL	0	NULL	tandem-mass spectroscopy 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The determination of serum choline concentrations was carried out by tandem-mass spectroscopy .
	manualset3
220579	1	420545	7	NULL	NULL	0	NULL	Ambulatory surgical gynecology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Ambulatory surgical gynecology : an overview .
	manualset3
220580	2	420545	7	NULL	NULL	0	NULL	overview 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ambulatory surgical gynecology : an overview .
	manualset3
220581	1	420546	7	NULL	NULL	0	NULL	 effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of 5-HT was mimicked by 1-phenylbiguanide , a 5-HT3 receptor agonist , but not by 8-hydroxy-2 - ( di-n-propylamino ) tetralin , a 5-HT1A receptor agonist .
	manualset3
220582	2	420546	7	NULL	NULL	0	NULL	 5-HT	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of 5-HT was mimicked by 1-phenylbiguanide , a 5-HT3 receptor agonist , but not by 8-hydroxy-2 - ( di-n-propylamino ) tetralin , a 5-HT1A receptor agonist .
	manualset3
220583	3	420546	7	NULL	NULL	0	NULL	1-phenylbiguanide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of 5-HT was mimicked by 1-phenylbiguanide , a 5-HT3 receptor agonist , but not by 8-hydroxy-2 - ( di-n-propylamino ) tetralin , a 5-HT1A receptor agonist .
	manualset3
220584	4	420546	7	NULL	NULL	0	NULL	 5-HT3 receptor agonist 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of 5-HT was mimicked by 1-phenylbiguanide , a 5-HT3 receptor agonist , but not by 8-hydroxy-2 - ( di-n-propylamino ) tetralin , a 5-HT1A receptor agonist .
	manualset3
220585	5	420546	7	NULL	NULL	0	NULL	8-hydroxy-2 - ( di-n-propylamino ) tetralin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of 5-HT was mimicked by 1-phenylbiguanide , a 5-HT3 receptor agonist , but not by 8-hydroxy-2 - ( di-n-propylamino ) tetralin , a 5-HT1A receptor agonist .
	manualset3
220586	6	420546	7	NULL	NULL	0	NULL	 5-HT1A receptor agonist 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of 5-HT was mimicked by 1-phenylbiguanide , a 5-HT3 receptor agonist , but not by 8-hydroxy-2 - ( di-n-propylamino ) tetralin , a 5-HT1A receptor agonist .
	manualset3
220587	1	420547	7	NULL	NULL	0	NULL	Past approaches	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Past approaches have been largely empirical and generally used a single type of adjuvant , such as aluminium salts or emulsions .
	manualset3
220588	2	420547	7	NULL	NULL	0	NULL	single type	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Past approaches have been largely empirical and generally used a single type of adjuvant , such as aluminium salts or emulsions .
	manualset3
220589	3	420547	7	NULL	NULL	0	NULL	adjuvant 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Past approaches have been largely empirical and generally used a single type of adjuvant , such as aluminium salts or emulsions .
	manualset3
220590	4	420547	7	NULL	NULL	0	NULL	aluminium salts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Past approaches have been largely empirical and generally used a single type of adjuvant , such as aluminium salts or emulsions .
	manualset3
220591	5	420547	7	NULL	NULL	0	NULL	emulsions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Past approaches have been largely empirical and generally used a single type of adjuvant , such as aluminium salts or emulsions .
	manualset3
220592	1	420548	7	NULL	NULL	0	NULL	contraction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The contraction was more dependent on concentration of extracellular Ca2 + than CCh-induced contraction .
	manualset3
220593	2	420548	7	NULL	NULL	0	NULL	concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The contraction was more dependent on concentration of extracellular Ca2 + than CCh-induced contraction .
	manualset3
220594	3	420548	7	NULL	NULL	0	NULL	extracellular Ca2 +	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The contraction was more dependent on concentration of extracellular Ca2 + than CCh-induced contraction .
	manualset3
220595	4	420548	7	NULL	NULL	0	NULL	CCh-induced contraction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The contraction was more dependent on concentration of extracellular Ca2 + than CCh-induced contraction .
	manualset3
220596	1	420549	7	NULL	NULL	0	NULL	fluid shift	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This fluid shift from the vasculature into the interstitium probably prevented an even greater rise in arterial pressure .
	manualset3
220597	2	420549	7	NULL	NULL	0	NULL	 vasculature	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This fluid shift from the vasculature into the interstitium probably prevented an even greater rise in arterial pressure .
	manualset3
220598	3	420549	7	NULL	NULL	0	NULL	interstitium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This fluid shift from the vasculature into the interstitium probably prevented an even greater rise in arterial pressure .
	manualset3
220599	4	420549	7	NULL	NULL	0	NULL	greater rise	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This fluid shift from the vasculature into the interstitium probably prevented an even greater rise in arterial pressure .
	manualset3
220600	5	420549	7	NULL	NULL	0	NULL	arterial pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This fluid shift from the vasculature into the interstitium probably prevented an even greater rise in arterial pressure .
	manualset3
220601	1	420550	7	NULL	NULL	NULL	NULL	Radiological examination	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Radiological examination showed ossification of the transverse ligament of the atlas ( TLA ) and severe stenosis of the upper cervical canal .
	manualset3
220602	2	420550	7	NULL	NULL	NULL	NULL	ossification 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Radiological examination showed ossification of the transverse ligament of the atlas ( TLA ) and severe stenosis of the upper cervical canal .
	manualset3
220603	3	420550	7	NULL	NULL	NULL	NULL	 transverse ligament of the atlas ( TLA )	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Radiological examination showed ossification of the transverse ligament of the atlas ( TLA ) and severe stenosis of the upper cervical canal .
	manualset3
220604	4	420550	7	NULL	NULL	0	NULL	severe stenosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiological examination showed ossification of the transverse ligament of the atlas ( TLA ) and severe stenosis of the upper cervical canal .
	manualset3
220605	5	420550	7	NULL	NULL	0	NULL	upper cervical canal 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiological examination showed ossification of the transverse ligament of the atlas ( TLA ) and severe stenosis of the upper cervical canal .
	manualset3
220606	1	420551	7	NULL	NULL	0	NULL	biorhythm	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A biorhythm in bone growth in the rabbit .
	manualset3
220607	2	420551	7	NULL	NULL	0	NULL	bone growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A biorhythm in bone growth in the rabbit .
	manualset3
220608	3	420551	7	NULL	NULL	0	NULL	 rabbit	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A biorhythm in bone growth in the rabbit .
	manualset3
220609	1	420552	7	NULL	NULL	0	NULL	procedure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This procedure was repeated two more times to achieve a higher degree of multiwalled carbon nanotube functionalization .
	manualset3
220610	2	420552	7	NULL	NULL	0	NULL	two more times 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This procedure was repeated two more times to achieve a higher degree of multiwalled carbon nanotube functionalization .
	manualset3
220611	3	420552	7	NULL	NULL	0	NULL	higher degree	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This procedure was repeated two more times to achieve a higher degree of multiwalled carbon nanotube functionalization .
	manualset3
220612	4	420552	7	NULL	NULL	0	NULL	multiwalled carbon nanotube functionalization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This procedure was repeated two more times to achieve a higher degree of multiwalled carbon nanotube functionalization .
	manualset3
220613	1	420553	7	NULL	NULL	0	NULL	supposition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The supposition that delusions are a variety of belief has itself been questioned .
	manualset3
220614	2	420553	7	NULL	NULL	0	NULL	delusions 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The supposition that delusions are a variety of belief has itself been questioned .
	manualset3
220615	3	420553	7	NULL	NULL	0	NULL	belief 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The supposition that delusions are a variety of belief has itself been questioned .
	manualset3
220616	1	420554	7	NULL	NULL	0	NULL	Hormonal therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Hormonal therapy and uterine steroid receptors in myoma ) .
	manualset3
220617	2	420554	7	NULL	NULL	0	NULL	uterine steroid receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Hormonal therapy and uterine steroid receptors in myoma ) .
	manualset3
220618	3	420554	7	NULL	NULL	0	NULL	myoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Hormonal therapy and uterine steroid receptors in myoma ) .
	manualset3
220619	1	420555	7	NULL	NULL	0	NULL	factor of 100	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , a factor of 100 between the EC/LC50 of acute toxicity and NOEC of prolonged toxicity is scientifically justified .
	manualset3
220620	2	420555	7	NULL	NULL	0	NULL	EC/LC50	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , a factor of 100 between the EC/LC50 of acute toxicity and NOEC of prolonged toxicity is scientifically justified .
	manualset3
220621	3	420555	7	NULL	NULL	0	NULL	acute toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , a factor of 100 between the EC/LC50 of acute toxicity and NOEC of prolonged toxicity is scientifically justified .
	manualset3
220622	4	420555	7	NULL	NULL	0	NULL	NOEC 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , a factor of 100 between the EC/LC50 of acute toxicity and NOEC of prolonged toxicity is scientifically justified .
	manualset3
220623	5	420555	7	NULL	NULL	0	NULL	prolonged toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In general , a factor of 100 between the EC/LC50 of acute toxicity and NOEC of prolonged toxicity is scientifically justified .
	manualset3
220624	1	420556	7	NULL	NULL	0	NULL	Ten anthracyclines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten anthracyclines , including doxorubicin ( DX ) and daunorubicin ( DNR ) , and eight analogs with modifications in structure or stereochemistry of the aglycone and/or the aminosugar moiety were simultaneously tested in serial vitro titration studies against human adenocarcinomas in the human tumor stem cell assay .
	manualset3
220625	2	420556	7	NULL	NULL	0	NULL	doxorubicin ( DX )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten anthracyclines , including doxorubicin ( DX ) and daunorubicin ( DNR ) , and eight analogs with modifications in structure or stereochemistry of the aglycone and/or the aminosugar moiety were simultaneously tested in serial vitro titration studies against human adenocarcinomas in the human tumor stem cell assay .
	manualset3
220626	3	420556	7	NULL	NULL	0	NULL	daunorubicin ( DNR )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten anthracyclines , including doxorubicin ( DX ) and daunorubicin ( DNR ) , and eight analogs with modifications in structure or stereochemistry of the aglycone and/or the aminosugar moiety were simultaneously tested in serial vitro titration studies against human adenocarcinomas in the human tumor stem cell assay .
	manualset3
220627	4	420556	7	NULL	NULL	0	NULL	eight analogs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten anthracyclines , including doxorubicin ( DX ) and daunorubicin ( DNR ) , and eight analogs with modifications in structure or stereochemistry of the aglycone and/or the aminosugar moiety were simultaneously tested in serial vitro titration studies against human adenocarcinomas in the human tumor stem cell assay .
	manualset3
220628	5	420556	7	NULL	NULL	0	NULL	modifications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten anthracyclines , including doxorubicin ( DX ) and daunorubicin ( DNR ) , and eight analogs with modifications in structure or stereochemistry of the aglycone and/or the aminosugar moiety were simultaneously tested in serial vitro titration studies against human adenocarcinomas in the human tumor stem cell assay .
	manualset3
220629	6	420556	7	NULL	NULL	0	NULL	 structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten anthracyclines , including doxorubicin ( DX ) and daunorubicin ( DNR ) , and eight analogs with modifications in structure or stereochemistry of the aglycone and/or the aminosugar moiety were simultaneously tested in serial vitro titration studies against human adenocarcinomas in the human tumor stem cell assay .
	manualset3
220630	7	420556	7	NULL	NULL	0	NULL	stereochemistry	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten anthracyclines , including doxorubicin ( DX ) and daunorubicin ( DNR ) , and eight analogs with modifications in structure or stereochemistry of the aglycone and/or the aminosugar moiety were simultaneously tested in serial vitro titration studies against human adenocarcinomas in the human tumor stem cell assay .
	manualset3
220631	8	420556	7	NULL	NULL	0	NULL	aglycone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten anthracyclines , including doxorubicin ( DX ) and daunorubicin ( DNR ) , and eight analogs with modifications in structure or stereochemistry of the aglycone and/or the aminosugar moiety were simultaneously tested in serial vitro titration studies against human adenocarcinomas in the human tumor stem cell assay .
	manualset3
220632	9	420556	7	NULL	NULL	0	NULL	aminosugar moiety 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten anthracyclines , including doxorubicin ( DX ) and daunorubicin ( DNR ) , and eight analogs with modifications in structure or stereochemistry of the aglycone and/or the aminosugar moiety were simultaneously tested in serial vitro titration studies against human adenocarcinomas in the human tumor stem cell assay .
	manualset3
220633	10	420556	7	NULL	NULL	0	NULL	serial vitro titration studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten anthracyclines , including doxorubicin ( DX ) and daunorubicin ( DNR ) , and eight analogs with modifications in structure or stereochemistry of the aglycone and/or the aminosugar moiety were simultaneously tested in serial vitro titration studies against human adenocarcinomas in the human tumor stem cell assay .
	manualset3
220634	11	420556	7	NULL	NULL	0	NULL	human adenocarcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten anthracyclines , including doxorubicin ( DX ) and daunorubicin ( DNR ) , and eight analogs with modifications in structure or stereochemistry of the aglycone and/or the aminosugar moiety were simultaneously tested in serial vitro titration studies against human adenocarcinomas in the human tumor stem cell assay .
	manualset3
220635	12	420556	7	NULL	NULL	0	NULL	 human tumor stem cell assay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten anthracyclines , including doxorubicin ( DX ) and daunorubicin ( DNR ) , and eight analogs with modifications in structure or stereochemistry of the aglycone and/or the aminosugar moiety were simultaneously tested in serial vitro titration studies against human adenocarcinomas in the human tumor stem cell assay .
	manualset3
220641	1	420558	7	NULL	NULL	0	NULL	 observations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations confirm that the coupling between the ribs and the lung varies from the top to the base of the ribcage .
	manualset3
220642	2	420558	7	NULL	NULL	0	NULL	coupling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations confirm that the coupling between the ribs and the lung varies from the top to the base of the ribcage .
	manualset3
220643	3	420558	7	NULL	NULL	0	NULL	ribs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations confirm that the coupling between the ribs and the lung varies from the top to the base of the ribcage .
	manualset3
220644	4	420558	7	NULL	NULL	0	NULL	 lung 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations confirm that the coupling between the ribs and the lung varies from the top to the base of the ribcage .
	manualset3
220645	5	420558	7	NULL	NULL	0	NULL	base of the ribcage	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These observations confirm that the coupling between the ribs and the lung varies from the top to the base of the ribcage .
	manualset3
220646	1	420559	7	NULL	NULL	0	NULL	Independent occurrence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Independent occurrence of this in 2 locations in the opposite hemifields would be evidence of attention splitting .
	manualset3
220647	2	420559	7	NULL	NULL	0	NULL	2 locations 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Independent occurrence of this in 2 locations in the opposite hemifields would be evidence of attention splitting .
	manualset3
220648	3	420559	7	NULL	NULL	0	NULL	opposite hemifields	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Independent occurrence of this in 2 locations in the opposite hemifields would be evidence of attention splitting .
	manualset3
220649	4	420559	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Independent occurrence of this in 2 locations in the opposite hemifields would be evidence of attention splitting .
	manualset3
220650	5	420559	7	NULL	NULL	0	NULL	attention splitting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Independent occurrence of this in 2 locations in the opposite hemifields would be evidence of attention splitting .
	manualset3
220651	1	420560	7	NULL	NULL	0	NULL	Amer2 Protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Amer2 Protein Is a Novel Negative Regulator of Wnt / - Catenin Signaling Involved in Neuroectodermal Patterning .
	manualset3
220652	2	420560	7	NULL	NULL	0	NULL	Novel Negative Regulator	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Amer2 Protein Is a Novel Negative Regulator of Wnt / - Catenin Signaling Involved in Neuroectodermal Patterning .
	manualset3
220653	3	420560	7	NULL	NULL	0	NULL	 Wnt / - Catenin Signaling 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Amer2 Protein Is a Novel Negative Regulator of Wnt / - Catenin Signaling Involved in Neuroectodermal Patterning .
	manualset3
220654	4	420560	7	NULL	NULL	NULL	NULL	Neuroectodermal Patterning 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Amer2 Protein Is a Novel Negative Regulator of Wnt / - Catenin Signaling Involved in Neuroectodermal Patterning .
	manualset3
220655	1	420561	7	NULL	NULL	0	NULL	Biotechnology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Biotechnology and microbiology -- have reached the end of the line ?
	manualset3
220656	2	420561	7	NULL	NULL	0	NULL	microbiology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Biotechnology and microbiology -- have reached the end of the line ?
	manualset3
220657	3	420561	7	NULL	NULL	0	NULL	end of the line 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Biotechnology and microbiology -- have reached the end of the line ?
	manualset3
220658	1	420562	7	NULL	NULL	0	NULL	Clinical relevance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical relevance of `` late '' in the management of late relapse after treatment for a germ cell tumor .
	manualset3
220659	2	420562	7	NULL	NULL	0	NULL	 `` late '' 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical relevance of `` late '' in the management of late relapse after treatment for a germ cell tumor .
	manualset3
220660	3	420562	7	NULL	NULL	0	NULL	management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical relevance of `` late '' in the management of late relapse after treatment for a germ cell tumor .
	manualset3
220661	4	420562	7	NULL	NULL	0	NULL	late relapse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical relevance of `` late '' in the management of late relapse after treatment for a germ cell tumor .
	manualset3
220662	5	420562	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical relevance of `` late '' in the management of late relapse after treatment for a germ cell tumor .
	manualset3
220663	6	420562	7	NULL	NULL	0	NULL	 germ cell tumor	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical relevance of `` late '' in the management of late relapse after treatment for a germ cell tumor .
	manualset3
220664	1	420563	7	NULL	NULL	0	NULL	 data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data confirm the hypothesis of a direct action of the drug on T lymphocytes , but are also consistent with its influence on B cells too , even though with an opposite effect .
	manualset3
220665	2	420563	7	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These data confirm the hypothesis of a direct action of the drug on T lymphocytes , but are also consistent with its influence on B cells too , even though with an opposite effect .
	manualset3
220666	3	420563	7	NULL	NULL	0	NULL	direct action	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data confirm the hypothesis of a direct action of the drug on T lymphocytes , but are also consistent with its influence on B cells too , even though with an opposite effect .
	manualset3
220667	4	420563	7	NULL	NULL	0	NULL	drug 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	These data confirm the hypothesis of a direct action of the drug on T lymphocytes , but are also consistent with its influence on B cells too , even though with an opposite effect .
	manualset3
220668	5	420563	7	NULL	NULL	0	NULL	T lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These data confirm the hypothesis of a direct action of the drug on T lymphocytes , but are also consistent with its influence on B cells too , even though with an opposite effect .
	manualset3
220669	6	420563	7	NULL	NULL	0	NULL	B cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These data confirm the hypothesis of a direct action of the drug on T lymphocytes , but are also consistent with its influence on B cells too , even though with an opposite effect .
	manualset3
220670	7	420563	7	NULL	NULL	0	NULL	 opposite effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These data confirm the hypothesis of a direct action of the drug on T lymphocytes , but are also consistent with its influence on B cells too , even though with an opposite effect .
	manualset3
220671	1	420564	7	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among patients with stable disease or disease progression , those with symptom improvement had significantly better overall survival than those without improvement .
	manualset3
220672	2	420564	7	NULL	NULL	0	NULL	 stable disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Among patients with stable disease or disease progression , those with symptom improvement had significantly better overall survival than those without improvement .
	manualset3
220673	3	420564	7	NULL	NULL	0	NULL	disease progression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among patients with stable disease or disease progression , those with symptom improvement had significantly better overall survival than those without improvement .
	manualset3
220674	4	420564	7	NULL	NULL	0	NULL	symptom improvement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among patients with stable disease or disease progression , those with symptom improvement had significantly better overall survival than those without improvement .
	manualset3
220675	5	420564	7	NULL	NULL	0	NULL	overall survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among patients with stable disease or disease progression , those with symptom improvement had significantly better overall survival than those without improvement .
	manualset3
220676	6	420564	7	NULL	NULL	0	NULL	improvement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among patients with stable disease or disease progression , those with symptom improvement had significantly better overall survival than those without improvement .
	manualset3
220677	1	420565	7	NULL	NULL	0	NULL	Interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions of oral coumarin anticoagulants .
	manualset3
220678	2	420565	7	NULL	NULL	0	NULL	oral coumarin anticoagulants	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions of oral coumarin anticoagulants .
	manualset3
220679	1	420566	7	NULL	NULL	0	NULL	daily number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The daily number of capsules of Pancrease varies from 4 to 57 .
	manualset3
220680	2	420566	7	NULL	NULL	0	NULL	capsules	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The daily number of capsules of Pancrease varies from 4 to 57 .
	manualset3
220681	3	420566	7	NULL	NULL	0	NULL	Pancrease	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The daily number of capsules of Pancrease varies from 4 to 57 .
	manualset3
220682	4	420566	7	NULL	NULL	0	NULL	4	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The daily number of capsules of Pancrease varies from 4 to 57 .
	manualset3
220683	5	420566	7	NULL	NULL	0	NULL	57	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The daily number of capsules of Pancrease varies from 4 to 57 .
	manualset3
220684	1	420567	7	NULL	NULL	0	NULL	13 boys	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( 13 boys , 8 girls ) was compared to a control group of 21 children matched on sex , age , and socioeconomic level using the Bender Visual-Motor Gestalt Test .
	manualset3
220685	2	420567	7	NULL	NULL	0	NULL	8 girls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( 13 boys , 8 girls ) was compared to a control group of 21 children matched on sex , age , and socioeconomic level using the Bender Visual-Motor Gestalt Test .
	manualset3
220686	3	420567	7	NULL	NULL	0	NULL	control group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( 13 boys , 8 girls ) was compared to a control group of 21 children matched on sex , age , and socioeconomic level using the Bender Visual-Motor Gestalt Test .
	manualset3
220687	4	420567	7	NULL	NULL	0	NULL	21 children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( 13 boys , 8 girls ) was compared to a control group of 21 children matched on sex , age , and socioeconomic level using the Bender Visual-Motor Gestalt Test .
	manualset3
220688	5	420567	7	NULL	NULL	0	NULL	sex	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( 13 boys , 8 girls ) was compared to a control group of 21 children matched on sex , age , and socioeconomic level using the Bender Visual-Motor Gestalt Test .
	manualset3
220689	6	420567	7	NULL	NULL	NULL	NULL	age	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( 13 boys , 8 girls ) was compared to a control group of 21 children matched on sex , age , and socioeconomic level using the Bender Visual-Motor Gestalt Test .
	manualset3
220690	7	420567	7	NULL	NULL	0	NULL	 socioeconomic level	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	( 13 boys , 8 girls ) was compared to a control group of 21 children matched on sex , age , and socioeconomic level using the Bender Visual-Motor Gestalt Test .
	manualset3
220691	8	420567	7	NULL	NULL	0	NULL	Bender Visual-Motor Gestalt Test	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( 13 boys , 8 girls ) was compared to a control group of 21 children matched on sex , age , and socioeconomic level using the Bender Visual-Motor Gestalt Test .
	manualset3
220692	1	420568	7	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We apply this to the study of the thermal expansivity of mixtures of 1-palmitoyl-2-oleoyl sn-glycero-3-phosphatidylcholine ( POPC ) and cholesterol as a function of composition and temperature .
	manualset3
220693	2	420568	7	NULL	NULL	0	NULL	 thermal expansivity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We apply this to the study of the thermal expansivity of mixtures of 1-palmitoyl-2-oleoyl sn-glycero-3-phosphatidylcholine ( POPC ) and cholesterol as a function of composition and temperature .
	manualset3
220694	3	420568	7	NULL	NULL	0	NULL	mixtures	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We apply this to the study of the thermal expansivity of mixtures of 1-palmitoyl-2-oleoyl sn-glycero-3-phosphatidylcholine ( POPC ) and cholesterol as a function of composition and temperature .
	manualset3
220695	4	420568	7	NULL	NULL	0	NULL	1-palmitoyl-2-oleoyl sn-glycero-3-phosphatidylcholine ( POPC )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We apply this to the study of the thermal expansivity of mixtures of 1-palmitoyl-2-oleoyl sn-glycero-3-phosphatidylcholine ( POPC ) and cholesterol as a function of composition and temperature .
	manualset3
220696	5	420568	7	NULL	NULL	0	NULL	cholesterol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We apply this to the study of the thermal expansivity of mixtures of 1-palmitoyl-2-oleoyl sn-glycero-3-phosphatidylcholine ( POPC ) and cholesterol as a function of composition and temperature .
	manualset3
220697	6	420568	7	NULL	NULL	0	NULL	function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We apply this to the study of the thermal expansivity of mixtures of 1-palmitoyl-2-oleoyl sn-glycero-3-phosphatidylcholine ( POPC ) and cholesterol as a function of composition and temperature .
	manualset3
220698	7	420568	7	NULL	NULL	0	NULL	composition	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We apply this to the study of the thermal expansivity of mixtures of 1-palmitoyl-2-oleoyl sn-glycero-3-phosphatidylcholine ( POPC ) and cholesterol as a function of composition and temperature .
	manualset3
220699	8	420568	7	NULL	NULL	0	NULL	temperature	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We apply this to the study of the thermal expansivity of mixtures of 1-palmitoyl-2-oleoyl sn-glycero-3-phosphatidylcholine ( POPC ) and cholesterol as a function of composition and temperature .
	manualset3
220700	1	420569	7	NULL	NULL	0	NULL	Dental caries	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Dental caries of permanent molars in school children in Slovakia ) .
	manualset3
220701	2	420569	7	NULL	NULL	0	NULL	permanent molars 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Dental caries of permanent molars in school children in Slovakia ) .
	manualset3
220702	3	420569	7	NULL	NULL	0	NULL	school children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Dental caries of permanent molars in school children in Slovakia ) .
	manualset3
220703	4	420569	7	NULL	NULL	0	NULL	Slovakia 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Dental caries of permanent molars in school children in Slovakia ) .
	manualset3
220704	1	420570	7	NULL	NULL	0	NULL	chains 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These chains are further extended into a three-dimensional network via O-HO hydrogen-bonding inter-actions and inter-chain - stacking inter-actions ( centroid-centroid distance = 3.662 ( 2 ) ) .
	manualset3
220705	2	420570	7	NULL	NULL	0	NULL	three-dimensional network 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These chains are further extended into a three-dimensional network via O-HO hydrogen-bonding inter-actions and inter-chain - stacking inter-actions ( centroid-centroid distance = 3.662 ( 2 ) ) .
	manualset3
220706	3	420570	7	NULL	NULL	0	NULL	O-HO hydrogen-bonding inter-actions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These chains are further extended into a three-dimensional network via O-HO hydrogen-bonding inter-actions and inter-chain - stacking inter-actions ( centroid-centroid distance = 3.662 ( 2 ) ) .
	manualset3
220707	4	420570	7	NULL	NULL	0	NULL	 inter-chain - stacking inter-actions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These chains are further extended into a three-dimensional network via O-HO hydrogen-bonding inter-actions and inter-chain - stacking inter-actions ( centroid-centroid distance = 3.662 ( 2 ) ) .
	manualset3
220708	5	420570	7	NULL	NULL	0	NULL	centroid-centroid distance	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These chains are further extended into a three-dimensional network via O-HO hydrogen-bonding inter-actions and inter-chain - stacking inter-actions ( centroid-centroid distance = 3.662 ( 2 ) ) .
	manualset3
220709	6	420570	7	NULL	NULL	0	NULL	 3.662 ( 2 ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These chains are further extended into a three-dimensional network via O-HO hydrogen-bonding inter-actions and inter-chain - stacking inter-actions ( centroid-centroid distance = 3.662 ( 2 ) ) .
	manualset3
220710	1	420571	7	NULL	NULL	0	NULL	state of polarization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It appears that any state of polarization can be produced , at least on the first harmonic , with a large total polarization rate and a potentially high polarization switching frequency .
	manualset3
220711	2	420571	7	NULL	NULL	0	NULL	 large total polarization rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It appears that any state of polarization can be produced , at least on the first harmonic , with a large total polarization rate and a potentially high polarization switching frequency .
	manualset3
220712	3	420571	7	NULL	NULL	0	NULL	high polarization switching frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It appears that any state of polarization can be produced , at least on the first harmonic , with a large total polarization rate and a potentially high polarization switching frequency .
	manualset3
220713	1	420572	7	NULL	NULL	0	NULL	case 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A case is presented of basilar impression secondary to osteogenesis imperfecta tarda , associated with hemifacial spasm and brain-stem compression syndrome .
	manualset3
220714	2	420572	7	NULL	NULL	0	NULL	basilar impression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A case is presented of basilar impression secondary to osteogenesis imperfecta tarda , associated with hemifacial spasm and brain-stem compression syndrome .
	manualset3
220715	3	420572	7	NULL	NULL	NULL	NULL	osteogenesis imperfecta tarda 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A case is presented of basilar impression secondary to osteogenesis imperfecta tarda , associated with hemifacial spasm and brain-stem compression syndrome .
	manualset3
220716	4	420572	7	NULL	NULL	0	NULL	hemifacial spasm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A case is presented of basilar impression secondary to osteogenesis imperfecta tarda , associated with hemifacial spasm and brain-stem compression syndrome .
	manualset3
220717	5	420572	7	NULL	NULL	0	NULL	brain-stem compression syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A case is presented of basilar impression secondary to osteogenesis imperfecta tarda , associated with hemifacial spasm and brain-stem compression syndrome .
	manualset3
220718	1	420573	7	NULL	NULL	0	NULL	ST elevation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	ST elevation in leads V1 to V4 mimicking anteroseptal myocardial infarction was recorded at admission and during episodes of chest pain later on .
	manualset3
220719	2	420573	7	NULL	NULL	0	NULL	 leads V1	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	ST elevation in leads V1 to V4 mimicking anteroseptal myocardial infarction was recorded at admission and during episodes of chest pain later on .
	manualset3
220720	3	420573	7	NULL	NULL	0	NULL	leads V4	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	ST elevation in leads V1 to V4 mimicking anteroseptal myocardial infarction was recorded at admission and during episodes of chest pain later on .
	manualset3
220721	4	420573	7	NULL	NULL	0	NULL	anteroseptal myocardial infarction	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	ST elevation in leads V1 to V4 mimicking anteroseptal myocardial infarction was recorded at admission and during episodes of chest pain later on .
	manualset3
220722	5	420573	7	NULL	NULL	0	NULL	admission	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	ST elevation in leads V1 to V4 mimicking anteroseptal myocardial infarction was recorded at admission and during episodes of chest pain later on .
	manualset3
220723	6	420573	7	NULL	NULL	0	NULL	episodes	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	ST elevation in leads V1 to V4 mimicking anteroseptal myocardial infarction was recorded at admission and during episodes of chest pain later on .
	manualset3
220724	7	420573	7	NULL	NULL	0	NULL	chest pain 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	ST elevation in leads V1 to V4 mimicking anteroseptal myocardial infarction was recorded at admission and during episodes of chest pain later on .
	manualset3
220725	1	420574	7	NULL	NULL	0	NULL	Dihydroxyfumarate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Dihydroxyfumarate can not be replaced by ascorbate H2O2 , NADH , cysteine or sulphite .
	manualset3
220726	2	420574	7	NULL	NULL	NULL	NULL	ascorbate H2O2	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dihydroxyfumarate can not be replaced by ascorbate H2O2 , NADH , cysteine or sulphite .
	manualset3
220727	3	420574	7	NULL	NULL	0	NULL	NADH	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Dihydroxyfumarate can not be replaced by ascorbate H2O2 , NADH , cysteine or sulphite .
	manualset3
220728	4	420574	7	NULL	NULL	0	NULL	cysteine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Dihydroxyfumarate can not be replaced by ascorbate H2O2 , NADH , cysteine or sulphite .
	manualset3
220729	5	420574	7	NULL	NULL	0	NULL	 sulphite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Dihydroxyfumarate can not be replaced by ascorbate H2O2 , NADH , cysteine or sulphite .
	manualset3
220730	1	420575	7	NULL	NULL	0	NULL	primary laryngeal histologic findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary laryngeal histologic findings of specimens from individuals with PDs with or without CFMs do not differ substantially from those from normal individuals ; however , individuals with PDs do appear to be somewhat more susceptible to intubation injury and other acquired laryngeal injury .
	manualset3
220731	2	420575	7	NULL	NULL	0	NULL	specimens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary laryngeal histologic findings of specimens from individuals with PDs with or without CFMs do not differ substantially from those from normal individuals ; however , individuals with PDs do appear to be somewhat more susceptible to intubation injury and other acquired laryngeal injury .
	manualset3
220732	3	420575	7	NULL	NULL	NULL	NULL	individuals 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The primary laryngeal histologic findings of specimens from individuals with PDs with or without CFMs do not differ substantially from those from normal individuals ; however , individuals with PDs do appear to be somewhat more susceptible to intubation injury and other acquired laryngeal injury .
	manualset3
220733	4	420575	7	NULL	NULL	0	NULL	PDs	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary laryngeal histologic findings of specimens from individuals with PDs with or without CFMs do not differ substantially from those from normal individuals ; however , individuals with PDs do appear to be somewhat more susceptible to intubation injury and other acquired laryngeal injury .
	manualset3
220734	5	420575	7	NULL	NULL	0	NULL	 CFMs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary laryngeal histologic findings of specimens from individuals with PDs with or without CFMs do not differ substantially from those from normal individuals ; however , individuals with PDs do appear to be somewhat more susceptible to intubation injury and other acquired laryngeal injury .
	manualset3
220735	6	420575	7	NULL	NULL	0	NULL	normal individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary laryngeal histologic findings of specimens from individuals with PDs with or without CFMs do not differ substantially from those from normal individuals ; however , individuals with PDs do appear to be somewhat more susceptible to intubation injury and other acquired laryngeal injury .
	manualset3
220736	7	420575	7	NULL	NULL	0	NULL	individuals 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary laryngeal histologic findings of specimens from individuals with PDs with or without CFMs do not differ substantially from those from normal individuals ; however , individuals with PDs do appear to be somewhat more susceptible to intubation injury and other acquired laryngeal injury .
	manualset3
220737	8	420575	7	NULL	NULL	0	NULL	PDs	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary laryngeal histologic findings of specimens from individuals with PDs with or without CFMs do not differ substantially from those from normal individuals ; however , individuals with PDs do appear to be somewhat more susceptible to intubation injury and other acquired laryngeal injury .
	manualset3
220738	9	420575	7	NULL	NULL	0	NULL	intubation injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary laryngeal histologic findings of specimens from individuals with PDs with or without CFMs do not differ substantially from those from normal individuals ; however , individuals with PDs do appear to be somewhat more susceptible to intubation injury and other acquired laryngeal injury .
	manualset3
220739	10	420575	7	NULL	NULL	0	NULL	acquired laryngeal injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The primary laryngeal histologic findings of specimens from individuals with PDs with or without CFMs do not differ substantially from those from normal individuals ; however , individuals with PDs do appear to be somewhat more susceptible to intubation injury and other acquired laryngeal injury .
	manualset3
220740	1	420576	7	NULL	NULL	0	NULL	generous allocation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The previous generous allocation of care has been replaced by a more restrictive approach .
	manualset3
220741	2	420576	7	NULL	NULL	0	NULL	care	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The previous generous allocation of care has been replaced by a more restrictive approach .
	manualset3
220742	3	420576	7	NULL	NULL	0	NULL	 restrictive approach	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The previous generous allocation of care has been replaced by a more restrictive approach .
	manualset3
220743	1	420577	7	NULL	NULL	0	NULL	A-fibre neurones	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Most A-fibre neurones with CGRP-LI had inflections on the falling phase of the somatic AP .
	manualset3
220744	2	420577	7	NULL	NULL	NULL	NULL	CGRP-LI 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Most A-fibre neurones with CGRP-LI had inflections on the falling phase of the somatic AP .
	manualset3
220745	3	420577	7	NULL	NULL	0	NULL	 falling phase	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Most A-fibre neurones with CGRP-LI had inflections on the falling phase of the somatic AP .
	manualset3
220746	4	420577	7	NULL	NULL	0	NULL	 somatic AP	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Most A-fibre neurones with CGRP-LI had inflections on the falling phase of the somatic AP .
	manualset3
220747	5	420577	7	NULL	NULL	0	NULL	inflections	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most A-fibre neurones with CGRP-LI had inflections on the falling phase of the somatic AP .
	manualset3
220748	1	420578	7	NULL	NULL	0	NULL	Regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of integrin alpha 5 beta 1 function by anti-integrin antibodies and divalent cations .
	manualset3
220749	2	420578	7	NULL	NULL	0	NULL	integrin alpha 5 beta 1 function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of integrin alpha 5 beta 1 function by anti-integrin antibodies and divalent cations .
	manualset3
220750	3	420578	7	NULL	NULL	0	NULL	anti-integrin antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of integrin alpha 5 beta 1 function by anti-integrin antibodies and divalent cations .
	manualset3
220751	4	420578	7	NULL	NULL	0	NULL	divalent cations	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Regulation of integrin alpha 5 beta 1 function by anti-integrin antibodies and divalent cations .
	manualset3
220752	1	420579	7	NULL	NULL	0	NULL	 effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect was measured for individual gold nanoparticles of a variety of sizes and for a variety of laser powers .
	manualset3
220753	2	420579	7	NULL	NULL	0	NULL	individual gold nanoparticles	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect was measured for individual gold nanoparticles of a variety of sizes and for a variety of laser powers .
	manualset3
220754	3	420579	7	NULL	NULL	0	NULL	sizes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect was measured for individual gold nanoparticles of a variety of sizes and for a variety of laser powers .
	manualset3
220755	4	420579	7	NULL	NULL	0	NULL	laser powers	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect was measured for individual gold nanoparticles of a variety of sizes and for a variety of laser powers .
	manualset3
220756	1	420580	7	NULL	NULL	NULL	NULL	Genetic polymorphism 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Genetic polymorphism resulting in interindividual and interethnic variation in xenobiotic metabolism is responsible for differences in the susceptibility to chemical-induced toxicity and carcinogenicity , allowing the identification of people at increased risk .
	manualset3
220757	2	420580	7	NULL	NULL	0	NULL	 interindividual variation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic polymorphism resulting in interindividual and interethnic variation in xenobiotic metabolism is responsible for differences in the susceptibility to chemical-induced toxicity and carcinogenicity , allowing the identification of people at increased risk .
	manualset3
220758	3	420580	7	NULL	NULL	0	NULL	interethnic variation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic polymorphism resulting in interindividual and interethnic variation in xenobiotic metabolism is responsible for differences in the susceptibility to chemical-induced toxicity and carcinogenicity , allowing the identification of people at increased risk .
	manualset3
220759	4	420580	7	NULL	NULL	0	NULL	xenobiotic metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic polymorphism resulting in interindividual and interethnic variation in xenobiotic metabolism is responsible for differences in the susceptibility to chemical-induced toxicity and carcinogenicity , allowing the identification of people at increased risk .
	manualset3
220760	5	420580	7	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic polymorphism resulting in interindividual and interethnic variation in xenobiotic metabolism is responsible for differences in the susceptibility to chemical-induced toxicity and carcinogenicity , allowing the identification of people at increased risk .
	manualset3
220761	6	420580	7	NULL	NULL	0	NULL	susceptibility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic polymorphism resulting in interindividual and interethnic variation in xenobiotic metabolism is responsible for differences in the susceptibility to chemical-induced toxicity and carcinogenicity , allowing the identification of people at increased risk .
	manualset3
220762	7	420580	7	NULL	NULL	0	NULL	chemical-induced toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic polymorphism resulting in interindividual and interethnic variation in xenobiotic metabolism is responsible for differences in the susceptibility to chemical-induced toxicity and carcinogenicity , allowing the identification of people at increased risk .
	manualset3
220763	8	420580	7	NULL	NULL	0	NULL	carcinogenicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic polymorphism resulting in interindividual and interethnic variation in xenobiotic metabolism is responsible for differences in the susceptibility to chemical-induced toxicity and carcinogenicity , allowing the identification of people at increased risk .
	manualset3
220764	9	420580	7	NULL	NULL	0	NULL	identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic polymorphism resulting in interindividual and interethnic variation in xenobiotic metabolism is responsible for differences in the susceptibility to chemical-induced toxicity and carcinogenicity , allowing the identification of people at increased risk .
	manualset3
220765	10	420580	7	NULL	NULL	0	NULL	people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic polymorphism resulting in interindividual and interethnic variation in xenobiotic metabolism is responsible for differences in the susceptibility to chemical-induced toxicity and carcinogenicity , allowing the identification of people at increased risk .
	manualset3
220766	11	420580	7	NULL	NULL	0	NULL	 increased risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic polymorphism resulting in interindividual and interethnic variation in xenobiotic metabolism is responsible for differences in the susceptibility to chemical-induced toxicity and carcinogenicity , allowing the identification of people at increased risk .
	manualset3
220767	1	420581	7	NULL	NULL	0	NULL	Patient cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient cultures treated by FudR presented a threefold increase of chromosome type alterations respect to chromatid ones .
	manualset3
220768	2	420581	7	NULL	NULL	NULL	NULL	FudR	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patient cultures treated by FudR presented a threefold increase of chromosome type alterations respect to chromatid ones .
	manualset3
220769	3	420581	7	NULL	NULL	0	NULL	threefold increase	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient cultures treated by FudR presented a threefold increase of chromosome type alterations respect to chromatid ones .
	manualset3
220770	4	420581	7	NULL	NULL	0	NULL	chromosome type alterations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient cultures treated by FudR presented a threefold increase of chromosome type alterations respect to chromatid ones .
	manualset3
220771	5	420581	7	NULL	NULL	0	NULL	chromatid ones	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient cultures treated by FudR presented a threefold increase of chromosome type alterations respect to chromatid ones .
	manualset3
220772	1	420582	7	NULL	NULL	0	NULL	Fractionation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractionation of polarized cells incubated with 125I-Shiga toxin showed that the transport of toxin to the Golgi apparatus was equally efficient from both poles of the cells .
	manualset3
220773	2	420582	7	NULL	NULL	0	NULL	polarized cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractionation of polarized cells incubated with 125I-Shiga toxin showed that the transport of toxin to the Golgi apparatus was equally efficient from both poles of the cells .
	manualset3
220774	3	420582	7	NULL	NULL	0	NULL	125I-Shiga toxin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractionation of polarized cells incubated with 125I-Shiga toxin showed that the transport of toxin to the Golgi apparatus was equally efficient from both poles of the cells .
	manualset3
220775	4	420582	7	NULL	NULL	0	NULL	transport	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractionation of polarized cells incubated with 125I-Shiga toxin showed that the transport of toxin to the Golgi apparatus was equally efficient from both poles of the cells .
	manualset3
220776	5	420582	7	NULL	NULL	0	NULL	 toxin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractionation of polarized cells incubated with 125I-Shiga toxin showed that the transport of toxin to the Golgi apparatus was equally efficient from both poles of the cells .
	manualset3
220777	6	420582	7	NULL	NULL	0	NULL	Golgi apparatus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractionation of polarized cells incubated with 125I-Shiga toxin showed that the transport of toxin to the Golgi apparatus was equally efficient from both poles of the cells .
	manualset3
220778	7	420582	7	NULL	NULL	0	NULL	 poles of the cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractionation of polarized cells incubated with 125I-Shiga toxin showed that the transport of toxin to the Golgi apparatus was equally efficient from both poles of the cells .
	manualset3
220779	1	420583	7	NULL	NULL	0	NULL	Restricted fed cows 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Restricted fed cows had slightly different acute fever responses and significantly increased heart and respiration rates than ad libitum fed cows .
	manualset3
220780	2	420583	7	NULL	NULL	0	NULL	acute fever responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Restricted fed cows had slightly different acute fever responses and significantly increased heart and respiration rates than ad libitum fed cows .
	manualset3
220781	3	420583	7	NULL	NULL	0	NULL	increased heart rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Restricted fed cows had slightly different acute fever responses and significantly increased heart and respiration rates than ad libitum fed cows .
	manualset3
220782	4	420583	7	NULL	NULL	0	NULL	respiration rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Restricted fed cows had slightly different acute fever responses and significantly increased heart and respiration rates than ad libitum fed cows .
	manualset3
220783	5	420583	7	NULL	NULL	0	NULL	ad libitum fed cows	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Restricted fed cows had slightly different acute fever responses and significantly increased heart and respiration rates than ad libitum fed cows .
	manualset3
220784	1	420584	7	NULL	NULL	0	NULL	Interleukin-6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-6 in aging and chronic disease : a magnificent pathway .
	manualset3
220785	2	420584	7	NULL	NULL	0	NULL	aging	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-6 in aging and chronic disease : a magnificent pathway .
	manualset3
220786	3	420584	7	NULL	NULL	0	NULL	chronic disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-6 in aging and chronic disease : a magnificent pathway .
	manualset3
220787	4	420584	7	NULL	NULL	0	NULL	magnificent pathway	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interleukin-6 in aging and chronic disease : a magnificent pathway .
	manualset3
220788	1	420585	7	NULL	NULL	0	NULL	incidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence , type and heterozygosity of the c-K-ras gene mutation showed no discrepancies between the original xenografts and the established cell lines .
	manualset3
220789	2	420585	7	NULL	NULL	0	NULL	type	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence , type and heterozygosity of the c-K-ras gene mutation showed no discrepancies between the original xenografts and the established cell lines .
	manualset3
220790	3	420585	7	NULL	NULL	0	NULL	heterozygosity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence , type and heterozygosity of the c-K-ras gene mutation showed no discrepancies between the original xenografts and the established cell lines .
	manualset3
220791	4	420585	7	NULL	NULL	0	NULL	c-K-ras gene mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence , type and heterozygosity of the c-K-ras gene mutation showed no discrepancies between the original xenografts and the established cell lines .
	manualset3
220792	5	420585	7	NULL	NULL	0	NULL	discrepancies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence , type and heterozygosity of the c-K-ras gene mutation showed no discrepancies between the original xenografts and the established cell lines .
	manualset3
220793	6	420585	7	NULL	NULL	0	NULL	original xenografts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence , type and heterozygosity of the c-K-ras gene mutation showed no discrepancies between the original xenografts and the established cell lines .
	manualset3
220794	7	420585	7	NULL	NULL	0	NULL	 cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The incidence , type and heterozygosity of the c-K-ras gene mutation showed no discrepancies between the original xenografts and the established cell lines .
	manualset3
220795	1	420586	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Such findings suggest that endocardial cells are more liable to accumulate Na ions intracellularly and K ions extracellularly when the Na , K-pump is suppressed by ouabain or K + - free perfusion , presumably due to lower activity of Na , K-ATPase in Endo compared to Epi .
	manualset3
220796	2	420586	7	NULL	NULL	0	NULL	endocardial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Such findings suggest that endocardial cells are more liable to accumulate Na ions intracellularly and K ions extracellularly when the Na , K-pump is suppressed by ouabain or K + - free perfusion , presumably due to lower activity of Na , K-ATPase in Endo compared to Epi .
	manualset3
220797	3	420586	7	NULL	NULL	0	NULL	Na ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Such findings suggest that endocardial cells are more liable to accumulate Na ions intracellularly and K ions extracellularly when the Na , K-pump is suppressed by ouabain or K + - free perfusion , presumably due to lower activity of Na , K-ATPase in Endo compared to Epi .
	manualset3
220798	4	420586	7	NULL	NULL	NULL	NULL	K ions	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Such findings suggest that endocardial cells are more liable to accumulate Na ions intracellularly and K ions extracellularly when the Na , K-pump is suppressed by ouabain or K + - free perfusion , presumably due to lower activity of Na , K-ATPase in Endo compared to Epi .
	manualset3
220800	6	420586	7	NULL	NULL	NULL	NULL	Na , K-pump	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Such findings suggest that endocardial cells are more liable to accumulate Na ions intracellularly and K ions extracellularly when the Na , K-pump is suppressed by ouabain or K + - free perfusion , presumably due to lower activity of Na , K-ATPase in Endo compared to Epi .
	manualset3
220801	7	420586	7	NULL	NULL	0	NULL	ouabain	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Such findings suggest that endocardial cells are more liable to accumulate Na ions intracellularly and K ions extracellularly when the Na , K-pump is suppressed by ouabain or K + - free perfusion , presumably due to lower activity of Na , K-ATPase in Endo compared to Epi .
	manualset3
220802	8	420586	7	NULL	NULL	0	NULL	K + - free perfusion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such findings suggest that endocardial cells are more liable to accumulate Na ions intracellularly and K ions extracellularly when the Na , K-pump is suppressed by ouabain or K + - free perfusion , presumably due to lower activity of Na , K-ATPase in Endo compared to Epi .
	manualset3
220803	9	420586	7	NULL	NULL	0	NULL	lower activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such findings suggest that endocardial cells are more liable to accumulate Na ions intracellularly and K ions extracellularly when the Na , K-pump is suppressed by ouabain or K + - free perfusion , presumably due to lower activity of Na , K-ATPase in Endo compared to Epi .
	manualset3
220804	10	420586	7	NULL	NULL	NULL	NULL	Na , K-ATPase	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Such findings suggest that endocardial cells are more liable to accumulate Na ions intracellularly and K ions extracellularly when the Na , K-pump is suppressed by ouabain or K + - free perfusion , presumably due to lower activity of Na , K-ATPase in Endo compared to Epi .
	manualset3
220805	11	420586	7	NULL	NULL	0	NULL	Endo	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Such findings suggest that endocardial cells are more liable to accumulate Na ions intracellularly and K ions extracellularly when the Na , K-pump is suppressed by ouabain or K + - free perfusion , presumably due to lower activity of Na , K-ATPase in Endo compared to Epi .
	manualset3
220806	12	420586	7	NULL	NULL	0	NULL	Epi	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Such findings suggest that endocardial cells are more liable to accumulate Na ions intracellularly and K ions extracellularly when the Na , K-pump is suppressed by ouabain or K + - free perfusion , presumably due to lower activity of Na , K-ATPase in Endo compared to Epi .
	manualset3
220807	1	420587	7	NULL	NULL	0	NULL	Amino-terminal sequencing 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino-terminal sequencing over the first 37 amino acids revealed that granulophysin was homologous to CD63 , melanoma antigen ME491 , and pltgp40 .
	manualset3
220808	2	420587	7	NULL	NULL	0	NULL	first 37 amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino-terminal sequencing over the first 37 amino acids revealed that granulophysin was homologous to CD63 , melanoma antigen ME491 , and pltgp40 .
	manualset3
220809	3	420587	7	NULL	NULL	0	NULL	granulophysin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino-terminal sequencing over the first 37 amino acids revealed that granulophysin was homologous to CD63 , melanoma antigen ME491 , and pltgp40 .
	manualset3
220810	4	420587	7	NULL	NULL	0	NULL	CD63 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino-terminal sequencing over the first 37 amino acids revealed that granulophysin was homologous to CD63 , melanoma antigen ME491 , and pltgp40 .
	manualset3
220811	5	420587	7	NULL	NULL	0	NULL	melanoma antigen ME491 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino-terminal sequencing over the first 37 amino acids revealed that granulophysin was homologous to CD63 , melanoma antigen ME491 , and pltgp40 .
	manualset3
220812	6	420587	7	NULL	NULL	0	NULL	pltgp40	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino-terminal sequencing over the first 37 amino acids revealed that granulophysin was homologous to CD63 , melanoma antigen ME491 , and pltgp40 .
	manualset3
220813	1	420588	7	NULL	NULL	0	NULL	Headache	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Headache , facial pain , dysphagia , burning sensations in the tongue , tinnitus , vertigo and voice and respiratory disorders were frequent complaints of 48 patients at our out-patient clinic between 1980 and 1985 .
	manualset3
220814	2	420588	7	NULL	NULL	0	NULL	facial pain 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Headache , facial pain , dysphagia , burning sensations in the tongue , tinnitus , vertigo and voice and respiratory disorders were frequent complaints of 48 patients at our out-patient clinic between 1980 and 1985 .
	manualset3
220815	3	420588	7	NULL	NULL	0	NULL	dysphagia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Headache , facial pain , dysphagia , burning sensations in the tongue , tinnitus , vertigo and voice and respiratory disorders were frequent complaints of 48 patients at our out-patient clinic between 1980 and 1985 .
	manualset3
220816	4	420588	7	NULL	NULL	0	NULL	burning sensations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Headache , facial pain , dysphagia , burning sensations in the tongue , tinnitus , vertigo and voice and respiratory disorders were frequent complaints of 48 patients at our out-patient clinic between 1980 and 1985 .
	manualset3
220817	5	420588	7	NULL	NULL	0	NULL	tongue	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Headache , facial pain , dysphagia , burning sensations in the tongue , tinnitus , vertigo and voice and respiratory disorders were frequent complaints of 48 patients at our out-patient clinic between 1980 and 1985 .
	manualset3
220818	6	420588	7	NULL	NULL	0	NULL	tinnitus 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Headache , facial pain , dysphagia , burning sensations in the tongue , tinnitus , vertigo and voice and respiratory disorders were frequent complaints of 48 patients at our out-patient clinic between 1980 and 1985 .
	manualset3
220819	7	420588	7	NULL	NULL	0	NULL	vertigo	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Headache , facial pain , dysphagia , burning sensations in the tongue , tinnitus , vertigo and voice and respiratory disorders were frequent complaints of 48 patients at our out-patient clinic between 1980 and 1985 .
	manualset3
220820	8	420588	7	NULL	NULL	0	NULL	voice disorder	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Headache , facial pain , dysphagia , burning sensations in the tongue , tinnitus , vertigo and voice and respiratory disorders were frequent complaints of 48 patients at our out-patient clinic between 1980 and 1985 .
	manualset3
220821	9	420588	7	NULL	NULL	0	NULL	respiratory disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Headache , facial pain , dysphagia , burning sensations in the tongue , tinnitus , vertigo and voice and respiratory disorders were frequent complaints of 48 patients at our out-patient clinic between 1980 and 1985 .
	manualset3
220822	10	420588	7	NULL	NULL	NULL	NULL	complaints	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Headache , facial pain , dysphagia , burning sensations in the tongue , tinnitus , vertigo and voice and respiratory disorders were frequent complaints of 48 patients at our out-patient clinic between 1980 and 1985 .
	manualset3
220823	11	420588	7	NULL	NULL	0	NULL	48 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Headache , facial pain , dysphagia , burning sensations in the tongue , tinnitus , vertigo and voice and respiratory disorders were frequent complaints of 48 patients at our out-patient clinic between 1980 and 1985 .
	manualset3
220824	12	420588	7	NULL	NULL	0	NULL	out-patient clinic 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Headache , facial pain , dysphagia , burning sensations in the tongue , tinnitus , vertigo and voice and respiratory disorders were frequent complaints of 48 patients at our out-patient clinic between 1980 and 1985 .
	manualset3
220825	13	420588	7	NULL	NULL	NULL	NULL	1980	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Headache , facial pain , dysphagia , burning sensations in the tongue , tinnitus , vertigo and voice and respiratory disorders were frequent complaints of 48 patients at our out-patient clinic between 1980 and 1985 .
	manualset3
220826	14	420588	7	NULL	NULL	NULL	NULL	 1985	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Headache , facial pain , dysphagia , burning sensations in the tongue , tinnitus , vertigo and voice and respiratory disorders were frequent complaints of 48 patients at our out-patient clinic between 1980 and 1985 .
	manualset3
220827	1	420589	7	NULL	NULL	0	NULL	method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This method was available to detect Pb/Cd or As ( III ) in water containing soil extracts .
	manualset3
220828	2	420589	7	NULL	NULL	0	NULL	Pb/Cd	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This method was available to detect Pb/Cd or As ( III ) in water containing soil extracts .
	manualset3
220829	3	420589	7	NULL	NULL	0	NULL	As ( III )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This method was available to detect Pb/Cd or As ( III ) in water containing soil extracts .
	manualset3
220830	4	420589	7	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This method was available to detect Pb/Cd or As ( III ) in water containing soil extracts .
	manualset3
220831	5	420589	7	NULL	NULL	0	NULL	soil extracts	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	This method was available to detect Pb/Cd or As ( III ) in water containing soil extracts .
	manualset3
220832	1	420590	7	NULL	NULL	0	NULL	cordotomies 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas some cordotomies , both in the current series and as reported in the literature , may affect these functions differentially , optimum pain relief seems to be obtained only when pinprick sensation is also abolished in the affected segments .
	manualset3
220833	2	420590	7	NULL	NULL	NULL	NULL	 current series 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Whereas some cordotomies , both in the current series and as reported in the literature , may affect these functions differentially , optimum pain relief seems to be obtained only when pinprick sensation is also abolished in the affected segments .
	manualset3
220834	3	420590	7	NULL	NULL	0	NULL	 literature 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas some cordotomies , both in the current series and as reported in the literature , may affect these functions differentially , optimum pain relief seems to be obtained only when pinprick sensation is also abolished in the affected segments .
	manualset3
220835	4	420590	7	NULL	NULL	0	NULL	functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas some cordotomies , both in the current series and as reported in the literature , may affect these functions differentially , optimum pain relief seems to be obtained only when pinprick sensation is also abolished in the affected segments .
	manualset3
220836	5	420590	7	NULL	NULL	0	NULL	optimum pain relief 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas some cordotomies , both in the current series and as reported in the literature , may affect these functions differentially , optimum pain relief seems to be obtained only when pinprick sensation is also abolished in the affected segments .
	manualset3
220837	6	420590	7	NULL	NULL	0	NULL	pinprick sensation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas some cordotomies , both in the current series and as reported in the literature , may affect these functions differentially , optimum pain relief seems to be obtained only when pinprick sensation is also abolished in the affected segments .
	manualset3
220838	7	420590	7	NULL	NULL	0	NULL	 affected segments	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Whereas some cordotomies , both in the current series and as reported in the literature , may affect these functions differentially , optimum pain relief seems to be obtained only when pinprick sensation is also abolished in the affected segments .
	manualset3
220839	1	420591	7	NULL	NULL	0	NULL	anti-Ro positive patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , it was found that anti-Ro positive patients with RA experienced a high frequency of side effects from penicillamine-D .
	manualset3
220840	2	420591	7	NULL	NULL	0	NULL	RA	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , it was found that anti-Ro positive patients with RA experienced a high frequency of side effects from penicillamine-D .
	manualset3
220841	3	420591	7	NULL	NULL	0	NULL	high frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , it was found that anti-Ro positive patients with RA experienced a high frequency of side effects from penicillamine-D .
	manualset3
220842	4	420591	7	NULL	NULL	0	NULL	side effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , it was found that anti-Ro positive patients with RA experienced a high frequency of side effects from penicillamine-D .
	manualset3
220843	5	420591	7	NULL	NULL	0	NULL	penicillamine-D 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , it was found that anti-Ro positive patients with RA experienced a high frequency of side effects from penicillamine-D .
	manualset3
220844	1	420592	7	NULL	NULL	0	NULL	high fat diet 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A high fat diet promotes the expression of FH .
	manualset3
220845	2	420592	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A high fat diet promotes the expression of FH .
	manualset3
220846	3	420592	7	NULL	NULL	0	NULL	FH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A high fat diet promotes the expression of FH .
	manualset3
220847	1	420593	7	NULL	NULL	0	NULL	Conclusions Morphologies	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions Morphologies of the glucose curve seem reflecting different metabolic phenotypes of insulin action and secretion , particularly when combined with morphologies of insulin curve or time of glucose peak .
	manualset3
220848	2	420593	7	NULL	NULL	0	NULL	glucose curve	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions Morphologies of the glucose curve seem reflecting different metabolic phenotypes of insulin action and secretion , particularly when combined with morphologies of insulin curve or time of glucose peak .
	manualset3
220849	3	420593	7	NULL	NULL	0	NULL	different metabolic phenotypes	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions Morphologies of the glucose curve seem reflecting different metabolic phenotypes of insulin action and secretion , particularly when combined with morphologies of insulin curve or time of glucose peak .
	manualset3
220850	4	420593	7	NULL	NULL	0	NULL	insulin action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions Morphologies of the glucose curve seem reflecting different metabolic phenotypes of insulin action and secretion , particularly when combined with morphologies of insulin curve or time of glucose peak .
	manualset3
220851	5	420593	7	NULL	NULL	0	NULL	secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions Morphologies of the glucose curve seem reflecting different metabolic phenotypes of insulin action and secretion , particularly when combined with morphologies of insulin curve or time of glucose peak .
	manualset3
220852	6	420593	7	NULL	NULL	0	NULL	morphologies	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions Morphologies of the glucose curve seem reflecting different metabolic phenotypes of insulin action and secretion , particularly when combined with morphologies of insulin curve or time of glucose peak .
	manualset3
220853	7	420593	7	NULL	NULL	0	NULL	insulin curve 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions Morphologies of the glucose curve seem reflecting different metabolic phenotypes of insulin action and secretion , particularly when combined with morphologies of insulin curve or time of glucose peak .
	manualset3
220854	8	420593	7	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions Morphologies of the glucose curve seem reflecting different metabolic phenotypes of insulin action and secretion , particularly when combined with morphologies of insulin curve or time of glucose peak .
	manualset3
220855	9	420593	7	NULL	NULL	0	NULL	glucose peak 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions Morphologies of the glucose curve seem reflecting different metabolic phenotypes of insulin action and secretion , particularly when combined with morphologies of insulin curve or time of glucose peak .
	manualset3
220856	1	420594	7	NULL	NULL	0	NULL	fourth part	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the fourth part of this review article , research on the topic of acupuncture and functional magnetic resonance imaging is described .
	manualset3
220857	2	420594	7	NULL	NULL	0	NULL	review article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In the fourth part of this review article , research on the topic of acupuncture and functional magnetic resonance imaging is described .
	manualset3
220858	3	420594	7	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the fourth part of this review article , research on the topic of acupuncture and functional magnetic resonance imaging is described .
	manualset3
220859	4	420594	7	NULL	NULL	0	NULL	 topic	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In the fourth part of this review article , research on the topic of acupuncture and functional magnetic resonance imaging is described .
	manualset3
220860	5	420594	7	NULL	NULL	0	NULL	acupuncture	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In the fourth part of this review article , research on the topic of acupuncture and functional magnetic resonance imaging is described .
	manualset3
220861	6	420594	7	NULL	NULL	0	NULL	functional magnetic resonance imaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the fourth part of this review article , research on the topic of acupuncture and functional magnetic resonance imaging is described .
	manualset3
220862	1	420595	7	NULL	NULL	0	NULL	Abstract Research 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Research has demonstrated that the jackknifing procedure for estimating ERP latencies ( J. Miller , T. Patterson , & R. Ulrich , 1998 ) yields more accurate estimates of differences between experimental conditions in ERP latency than other methods .
	manualset3
220863	2	420595	7	NULL	NULL	0	NULL	 jackknifing procedure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Research has demonstrated that the jackknifing procedure for estimating ERP latencies ( J. Miller , T. Patterson , & R. Ulrich , 1998 ) yields more accurate estimates of differences between experimental conditions in ERP latency than other methods .
	manualset3
220864	3	420595	7	NULL	NULL	0	NULL	ERP latencies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Research has demonstrated that the jackknifing procedure for estimating ERP latencies ( J. Miller , T. Patterson , & R. Ulrich , 1998 ) yields more accurate estimates of differences between experimental conditions in ERP latency than other methods .
	manualset3
220865	4	420595	7	NULL	NULL	0	NULL	J. Miller , T. Patterson , & R. Ulrich , 1998	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Research has demonstrated that the jackknifing procedure for estimating ERP latencies ( J. Miller , T. Patterson , & R. Ulrich , 1998 ) yields more accurate estimates of differences between experimental conditions in ERP latency than other methods .
	manualset3
220866	5	420595	7	NULL	NULL	0	NULL	accurate estimates	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Research has demonstrated that the jackknifing procedure for estimating ERP latencies ( J. Miller , T. Patterson , & R. Ulrich , 1998 ) yields more accurate estimates of differences between experimental conditions in ERP latency than other methods .
	manualset3
220867	6	420595	7	NULL	NULL	0	NULL	differences 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Research has demonstrated that the jackknifing procedure for estimating ERP latencies ( J. Miller , T. Patterson , & R. Ulrich , 1998 ) yields more accurate estimates of differences between experimental conditions in ERP latency than other methods .
	manualset3
220868	7	420595	7	NULL	NULL	0	NULL	experimental conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Research has demonstrated that the jackknifing procedure for estimating ERP latencies ( J. Miller , T. Patterson , & R. Ulrich , 1998 ) yields more accurate estimates of differences between experimental conditions in ERP latency than other methods .
	manualset3
220869	8	420595	7	NULL	NULL	0	NULL	ERP latency	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Research has demonstrated that the jackknifing procedure for estimating ERP latencies ( J. Miller , T. Patterson , & R. Ulrich , 1998 ) yields more accurate estimates of differences between experimental conditions in ERP latency than other methods .
	manualset3
220870	9	420595	7	NULL	NULL	0	NULL	methods	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Abstract Research has demonstrated that the jackknifing procedure for estimating ERP latencies ( J. Miller , T. Patterson , & R. Ulrich , 1998 ) yields more accurate estimates of differences between experimental conditions in ERP latency than other methods .
	manualset3
220871	1	420596	7	NULL	NULL	0	NULL	Characterization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Characterization of murine monoclonal anti-endothelial cell antibodies ( AECA ) produced by idiotypic manipulation with human AECA .
	manualset3
220872	2	420596	7	NULL	NULL	0	NULL	murine monoclonal anti-endothelial cell antibodies ( AECA ) 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Characterization of murine monoclonal anti-endothelial cell antibodies ( AECA ) produced by idiotypic manipulation with human AECA .
	manualset3
220873	3	420596	7	NULL	NULL	0	NULL	idiotypic manipulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Characterization of murine monoclonal anti-endothelial cell antibodies ( AECA ) produced by idiotypic manipulation with human AECA .
	manualset3
220874	4	420596	7	NULL	NULL	0	NULL	 human AECA	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Characterization of murine monoclonal anti-endothelial cell antibodies ( AECA ) produced by idiotypic manipulation with human AECA .
	manualset3
220875	1	420597	7	NULL	NULL	0	NULL	hypertonicity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was reported previously that hypertonicity exerted a dual , time-dependent effect on vasopressin-inducible aquaporin-2 ( AQP2 ) expression in immortalized mouse collecting duct principal cells ( mpkCCDcl4 ) .
	manualset3
220876	2	420597	7	NULL	NULL	0	NULL	dual , time-dependent effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was reported previously that hypertonicity exerted a dual , time-dependent effect on vasopressin-inducible aquaporin-2 ( AQP2 ) expression in immortalized mouse collecting duct principal cells ( mpkCCDcl4 ) .
	manualset3
220877	3	420597	7	NULL	NULL	0	NULL	vasopressin-inducible aquaporin-2 ( AQP2 ) expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was reported previously that hypertonicity exerted a dual , time-dependent effect on vasopressin-inducible aquaporin-2 ( AQP2 ) expression in immortalized mouse collecting duct principal cells ( mpkCCDcl4 ) .
	manualset3
220878	4	420597	7	NULL	NULL	0	NULL	 immortalized mouse collecting duct principal cells ( mpkCCDcl4 ) 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It was reported previously that hypertonicity exerted a dual , time-dependent effect on vasopressin-inducible aquaporin-2 ( AQP2 ) expression in immortalized mouse collecting duct principal cells ( mpkCCDcl4 ) .
	manualset3
220879	1	420598	7	NULL	NULL	0	NULL	disadvantages	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The disadvantages associated with systemic administration of PGs can be overcome by use of other routes of administration .
	manualset3
220880	2	420598	7	NULL	NULL	0	NULL	 systemic administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The disadvantages associated with systemic administration of PGs can be overcome by use of other routes of administration .
	manualset3
220881	3	420598	7	NULL	NULL	0	NULL	PGs	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The disadvantages associated with systemic administration of PGs can be overcome by use of other routes of administration .
	manualset3
220882	4	420598	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The disadvantages associated with systemic administration of PGs can be overcome by use of other routes of administration .
	manualset3
220883	5	420598	7	NULL	NULL	0	NULL	routes of administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The disadvantages associated with systemic administration of PGs can be overcome by use of other routes of administration .
	manualset3
220884	1	420599	7	NULL	NULL	0	NULL	Bone mineral density	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Bone mineral density of competitive male mountain and road cyclists .
	manualset3
220885	2	420599	7	NULL	NULL	0	NULL	competitive male mountain cyclists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Bone mineral density of competitive male mountain and road cyclists .
	manualset3
220886	3	420599	7	NULL	NULL	0	NULL	road cyclists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Bone mineral density of competitive male mountain and road cyclists .
	manualset3
220887	1	420600	7	NULL	NULL	0	NULL	active site 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The active site of MAO B consists of a 420 A ( 3 ) - hydrophobic substrate cavity interconnected to an entrance cavity of 290 A ( 3 ) .
	manualset3
220888	2	420600	7	NULL	NULL	0	NULL	MAO B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The active site of MAO B consists of a 420 A ( 3 ) - hydrophobic substrate cavity interconnected to an entrance cavity of 290 A ( 3 ) .
	manualset3
220889	3	420600	7	NULL	NULL	0	NULL	 420 A ( 3 ) - hydrophobic substrate cavity	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The active site of MAO B consists of a 420 A ( 3 ) - hydrophobic substrate cavity interconnected to an entrance cavity of 290 A ( 3 ) .
	manualset3
220890	4	420600	7	NULL	NULL	0	NULL	 entrance cavity 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The active site of MAO B consists of a 420 A ( 3 ) - hydrophobic substrate cavity interconnected to an entrance cavity of 290 A ( 3 ) .
	manualset3
220891	5	420600	7	NULL	NULL	0	NULL	290 A ( 3 )	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The active site of MAO B consists of a 420 A ( 3 ) - hydrophobic substrate cavity interconnected to an entrance cavity of 290 A ( 3 ) .
	manualset3
220892	1	420601	7	NULL	NULL	0	NULL	 reasons 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The reasons may be genetic differences in DNA repair .
	manualset3
220893	2	420601	7	NULL	NULL	0	NULL	genetic differences	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The reasons may be genetic differences in DNA repair .
	manualset3
220894	3	420601	7	NULL	NULL	0	NULL	DNA repair	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The reasons may be genetic differences in DNA repair .
	manualset3
220895	1	420602	7	NULL	NULL	0	NULL	Amino acid sequences	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino acid sequences of PrPc and PrPSc are identical , but their conformations are rather different ; PrPc rich in non beta-sheet vs. PrPSc rich in beta-sheet isoform .
	manualset3
220896	2	420602	7	NULL	NULL	0	NULL	PrPc	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino acid sequences of PrPc and PrPSc are identical , but their conformations are rather different ; PrPc rich in non beta-sheet vs. PrPSc rich in beta-sheet isoform .
	manualset3
220897	3	420602	7	NULL	NULL	0	NULL	PrPSc	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino acid sequences of PrPc and PrPSc are identical , but their conformations are rather different ; PrPc rich in non beta-sheet vs. PrPSc rich in beta-sheet isoform .
	manualset3
220898	4	420602	7	NULL	NULL	0	NULL	conformations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino acid sequences of PrPc and PrPSc are identical , but their conformations are rather different ; PrPc rich in non beta-sheet vs. PrPSc rich in beta-sheet isoform .
	manualset3
220899	5	420602	7	NULL	NULL	0	NULL	PrPc	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino acid sequences of PrPc and PrPSc are identical , but their conformations are rather different ; PrPc rich in non beta-sheet vs. PrPSc rich in beta-sheet isoform .
	manualset3
220900	6	420602	7	NULL	NULL	0	NULL	non beta-sheet	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino acid sequences of PrPc and PrPSc are identical , but their conformations are rather different ; PrPc rich in non beta-sheet vs. PrPSc rich in beta-sheet isoform .
	manualset3
220901	7	420602	7	NULL	NULL	0	NULL	PrPSc	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino acid sequences of PrPc and PrPSc are identical , but their conformations are rather different ; PrPc rich in non beta-sheet vs. PrPSc rich in beta-sheet isoform .
	manualset3
220902	8	420602	7	NULL	NULL	0	NULL	beta-sheet isoform	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino acid sequences of PrPc and PrPSc are identical , but their conformations are rather different ; PrPc rich in non beta-sheet vs. PrPSc rich in beta-sheet isoform .
	manualset3
220903	1	420603	7	NULL	NULL	0	NULL	ectopic fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar ectopic fibers were seen following transection of the optic nerve at the chiasm and after tectal ablation although the onset of these changes was slower than that seen after nerve resection .
	manualset3
220904	2	420603	7	NULL	NULL	0	NULL	transection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar ectopic fibers were seen following transection of the optic nerve at the chiasm and after tectal ablation although the onset of these changes was slower than that seen after nerve resection .
	manualset3
220905	3	420603	7	NULL	NULL	0	NULL	optic nerve	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar ectopic fibers were seen following transection of the optic nerve at the chiasm and after tectal ablation although the onset of these changes was slower than that seen after nerve resection .
	manualset3
220906	4	420603	7	NULL	NULL	NULL	NULL	chiasm	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Similar ectopic fibers were seen following transection of the optic nerve at the chiasm and after tectal ablation although the onset of these changes was slower than that seen after nerve resection .
	manualset3
220907	5	420603	7	NULL	NULL	0	NULL	tectal ablation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar ectopic fibers were seen following transection of the optic nerve at the chiasm and after tectal ablation although the onset of these changes was slower than that seen after nerve resection .
	manualset3
220908	6	420603	7	NULL	NULL	0	NULL	onset 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar ectopic fibers were seen following transection of the optic nerve at the chiasm and after tectal ablation although the onset of these changes was slower than that seen after nerve resection .
	manualset3
220909	7	420603	7	NULL	NULL	0	NULL	changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar ectopic fibers were seen following transection of the optic nerve at the chiasm and after tectal ablation although the onset of these changes was slower than that seen after nerve resection .
	manualset3
220910	8	420603	7	NULL	NULL	0	NULL	nerve resection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Similar ectopic fibers were seen following transection of the optic nerve at the chiasm and after tectal ablation although the onset of these changes was slower than that seen after nerve resection .
	manualset3
220912	1	420604	7	NULL	NULL	0	NULL	nephelometric method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A nephelometric method for the estimation of the binding power of thyroxine to blood proteins .
	manualset3
220913	2	420604	7	NULL	NULL	0	NULL	estimation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A nephelometric method for the estimation of the binding power of thyroxine to blood proteins .
	manualset3
220914	3	420604	7	NULL	NULL	NULL	NULL	binding power 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A nephelometric method for the estimation of the binding power of thyroxine to blood proteins .
	manualset3
220915	4	420604	7	NULL	NULL	0	NULL	thyroxine	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A nephelometric method for the estimation of the binding power of thyroxine to blood proteins .
	manualset3
220916	5	420604	7	NULL	NULL	0	NULL	blood proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A nephelometric method for the estimation of the binding power of thyroxine to blood proteins .
	manualset3
220917	1	420605	7	NULL	NULL	NULL	NULL	metal	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We demonstrate that the resulting deposited metal can be used to fabricate functional electrodes : The wet-deposited metal film can sustain patterning by photolithography down to micron-sized features required for MEMS and microfluidic applications , and its properties are suitable for operative electrodes used in a wide range of microfluidic applications for biological studies .
	manualset3
220918	2	420605	7	NULL	NULL	NULL	NULL	functional electrodes	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We demonstrate that the resulting deposited metal can be used to fabricate functional electrodes : The wet-deposited metal film can sustain patterning by photolithography down to micron-sized features required for MEMS and microfluidic applications , and its properties are suitable for operative electrodes used in a wide range of microfluidic applications for biological studies .
	manualset3
220919	3	420605	7	NULL	NULL	NULL	NULL	wet-deposited metal film	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We demonstrate that the resulting deposited metal can be used to fabricate functional electrodes : The wet-deposited metal film can sustain patterning by photolithography down to micron-sized features required for MEMS and microfluidic applications , and its properties are suitable for operative electrodes used in a wide range of microfluidic applications for biological studies .
	manualset3
220920	4	420605	7	NULL	NULL	0	NULL	photolithography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrate that the resulting deposited metal can be used to fabricate functional electrodes : The wet-deposited metal film can sustain patterning by photolithography down to micron-sized features required for MEMS and microfluidic applications , and its properties are suitable for operative electrodes used in a wide range of microfluidic applications for biological studies .
	manualset3
220921	5	420605	7	NULL	NULL	0	NULL	micron-sized features	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrate that the resulting deposited metal can be used to fabricate functional electrodes : The wet-deposited metal film can sustain patterning by photolithography down to micron-sized features required for MEMS and microfluidic applications , and its properties are suitable for operative electrodes used in a wide range of microfluidic applications for biological studies .
	manualset3
220922	6	420605	7	NULL	NULL	0	NULL	patterning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrate that the resulting deposited metal can be used to fabricate functional electrodes : The wet-deposited metal film can sustain patterning by photolithography down to micron-sized features required for MEMS and microfluidic applications , and its properties are suitable for operative electrodes used in a wide range of microfluidic applications for biological studies .
	manualset3
220923	7	420605	7	NULL	NULL	0	NULL	MEMS	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrate that the resulting deposited metal can be used to fabricate functional electrodes : The wet-deposited metal film can sustain patterning by photolithography down to micron-sized features required for MEMS and microfluidic applications , and its properties are suitable for operative electrodes used in a wide range of microfluidic applications for biological studies .
	manualset3
220924	8	420605	7	NULL	NULL	0	NULL	microfluidic applications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrate that the resulting deposited metal can be used to fabricate functional electrodes : The wet-deposited metal film can sustain patterning by photolithography down to micron-sized features required for MEMS and microfluidic applications , and its properties are suitable for operative electrodes used in a wide range of microfluidic applications for biological studies .
	manualset3
220925	9	420605	7	NULL	NULL	0	NULL	properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrate that the resulting deposited metal can be used to fabricate functional electrodes : The wet-deposited metal film can sustain patterning by photolithography down to micron-sized features required for MEMS and microfluidic applications , and its properties are suitable for operative electrodes used in a wide range of microfluidic applications for biological studies .
	manualset3
220926	10	420605	7	NULL	NULL	NULL	NULL	operative electrodes 	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We demonstrate that the resulting deposited metal can be used to fabricate functional electrodes : The wet-deposited metal film can sustain patterning by photolithography down to micron-sized features required for MEMS and microfluidic applications , and its properties are suitable for operative electrodes used in a wide range of microfluidic applications for biological studies .
	manualset3
220927	11	420605	7	NULL	NULL	0	NULL	wide range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrate that the resulting deposited metal can be used to fabricate functional electrodes : The wet-deposited metal film can sustain patterning by photolithography down to micron-sized features required for MEMS and microfluidic applications , and its properties are suitable for operative electrodes used in a wide range of microfluidic applications for biological studies .
	manualset3
220928	12	420605	7	NULL	NULL	0	NULL	microfluidic applications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrate that the resulting deposited metal can be used to fabricate functional electrodes : The wet-deposited metal film can sustain patterning by photolithography down to micron-sized features required for MEMS and microfluidic applications , and its properties are suitable for operative electrodes used in a wide range of microfluidic applications for biological studies .
	manualset3
220929	13	420605	7	NULL	NULL	0	NULL	biological studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrate that the resulting deposited metal can be used to fabricate functional electrodes : The wet-deposited metal film can sustain patterning by photolithography down to micron-sized features required for MEMS and microfluidic applications , and its properties are suitable for operative electrodes used in a wide range of microfluidic applications for biological studies .
	manualset3
221838	14	420605	7	NULL	NULL	0	NULL	patterning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrate that the resulting deposited metal can be used to fabricate functional electrodes : The wet-deposited metal film can sustain patterning by photolithography down to micron-sized features required for MEMS and microfluidic applications , and its properties are suitable for operative electrodes used in a wide range of microfluidic applications for biological studies .
	manualset3
220930	1	420606	7	NULL	NULL	0	NULL	Alternans	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Alternans , a beat-to-beat temporal alternation in the sequence of heartbeats , is a known precursor of the development of cardiac fibrillation , leading to sudden cardiac death .
	manualset3
220931	2	420606	7	NULL	NULL	0	NULL	beat-to-beat temporal alternation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Alternans , a beat-to-beat temporal alternation in the sequence of heartbeats , is a known precursor of the development of cardiac fibrillation , leading to sudden cardiac death .
	manualset3
220932	3	420606	7	NULL	NULL	0	NULL	sequence of heartbeats	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Alternans , a beat-to-beat temporal alternation in the sequence of heartbeats , is a known precursor of the development of cardiac fibrillation , leading to sudden cardiac death .
	manualset3
220933	4	420606	7	NULL	NULL	NULL	NULL	precursor	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Alternans , a beat-to-beat temporal alternation in the sequence of heartbeats , is a known precursor of the development of cardiac fibrillation , leading to sudden cardiac death .
	manualset3
220934	5	420606	7	NULL	NULL	0	NULL	 development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Alternans , a beat-to-beat temporal alternation in the sequence of heartbeats , is a known precursor of the development of cardiac fibrillation , leading to sudden cardiac death .
	manualset3
220935	6	420606	7	NULL	NULL	0	NULL	cardiac fibrillation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Alternans , a beat-to-beat temporal alternation in the sequence of heartbeats , is a known precursor of the development of cardiac fibrillation , leading to sudden cardiac death .
	manualset3
220936	7	420606	7	NULL	NULL	0	NULL	sudden cardiac death 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Alternans , a beat-to-beat temporal alternation in the sequence of heartbeats , is a known precursor of the development of cardiac fibrillation , leading to sudden cardiac death .
	manualset3
220937	1	420607	7	NULL	NULL	0	NULL	 results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained revealed that the SERT-BDNF interactions might moderate the level of anxiety and depression caused by caregiving status in parents of psychotic patients .
	manualset3
220938	2	420607	7	NULL	NULL	0	NULL	SERT-BDNF interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained revealed that the SERT-BDNF interactions might moderate the level of anxiety and depression caused by caregiving status in parents of psychotic patients .
	manualset3
220939	3	420607	7	NULL	NULL	0	NULL	level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained revealed that the SERT-BDNF interactions might moderate the level of anxiety and depression caused by caregiving status in parents of psychotic patients .
	manualset3
220940	4	420607	7	NULL	NULL	0	NULL	anxiety	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained revealed that the SERT-BDNF interactions might moderate the level of anxiety and depression caused by caregiving status in parents of psychotic patients .
	manualset3
220941	5	420607	7	NULL	NULL	0	NULL	depression	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained revealed that the SERT-BDNF interactions might moderate the level of anxiety and depression caused by caregiving status in parents of psychotic patients .
	manualset3
220942	6	420607	7	NULL	NULL	0	NULL	caregiving status	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained revealed that the SERT-BDNF interactions might moderate the level of anxiety and depression caused by caregiving status in parents of psychotic patients .
	manualset3
220943	7	420607	7	NULL	NULL	0	NULL	parents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained revealed that the SERT-BDNF interactions might moderate the level of anxiety and depression caused by caregiving status in parents of psychotic patients .
	manualset3
220944	8	420607	7	NULL	NULL	0	NULL	psychotic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained revealed that the SERT-BDNF interactions might moderate the level of anxiety and depression caused by caregiving status in parents of psychotic patients .
	manualset3
220945	1	420608	7	NULL	NULL	0	NULL	analogy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	By analogy with other neurosecretory systems , facilitation of calcium entry during the bursts may be responsible .
	manualset3
220946	2	420608	7	NULL	NULL	0	NULL	 neurosecretory systems	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	By analogy with other neurosecretory systems , facilitation of calcium entry during the bursts may be responsible .
	manualset3
220947	3	420608	7	NULL	NULL	0	NULL	facilitation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	By analogy with other neurosecretory systems , facilitation of calcium entry during the bursts may be responsible .
	manualset3
220948	4	420608	7	NULL	NULL	0	NULL	calcium entry	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	By analogy with other neurosecretory systems , facilitation of calcium entry during the bursts may be responsible .
	manualset3
220949	5	420608	7	NULL	NULL	0	NULL	 bursts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	By analogy with other neurosecretory systems , facilitation of calcium entry during the bursts may be responsible .
	manualset3
220950	1	420609	7	NULL	NULL	0	NULL	Acute episodes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute episodes of pain and acute chest syndrome ( ACS ) are the two leading causes of hospitalization .
	manualset3
220951	2	420609	7	NULL	NULL	0	NULL	pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute episodes of pain and acute chest syndrome ( ACS ) are the two leading causes of hospitalization .
	manualset3
220952	3	420609	7	NULL	NULL	0	NULL	acute chest syndrome ( ACS )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute episodes of pain and acute chest syndrome ( ACS ) are the two leading causes of hospitalization .
	manualset3
220953	4	420609	7	NULL	NULL	NULL	NULL	two leading causes	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Acute episodes of pain and acute chest syndrome ( ACS ) are the two leading causes of hospitalization .
	manualset3
220954	5	420609	7	NULL	NULL	0	NULL	hospitalization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute episodes of pain and acute chest syndrome ( ACS ) are the two leading causes of hospitalization .
	manualset3
220955	1	420610	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , adsorption capacity of chitosan to Acid Red 3R was found to be greatly enhanced in the presence of Cu2 + .
	manualset3
220956	2	420610	7	NULL	NULL	0	NULL	adsorption capacity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , adsorption capacity of chitosan to Acid Red 3R was found to be greatly enhanced in the presence of Cu2 + .
	manualset3
220957	3	420610	7	NULL	NULL	0	NULL	chitosan	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , adsorption capacity of chitosan to Acid Red 3R was found to be greatly enhanced in the presence of Cu2 + .
	manualset3
220958	4	420610	7	NULL	NULL	0	NULL	Acid Red 3R 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , adsorption capacity of chitosan to Acid Red 3R was found to be greatly enhanced in the presence of Cu2 + .
	manualset3
220959	5	420610	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , adsorption capacity of chitosan to Acid Red 3R was found to be greatly enhanced in the presence of Cu2 + .
	manualset3
220960	6	420610	7	NULL	NULL	0	NULL	Cu2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , adsorption capacity of chitosan to Acid Red 3R was found to be greatly enhanced in the presence of Cu2 + .
	manualset3
220961	1	420611	7	NULL	NULL	0	NULL	Amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino acids , particularly glutamate , gamma-aminobutyrate , aspartate and glycine , were released from rat brain slices on incubation with protoveratrine ( especially in a Ca ( 2 + ) - deficient medium ) or with ouabain or in the absence of glucose .
	manualset3
220962	2	420611	7	NULL	NULL	0	NULL	glutamate	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino acids , particularly glutamate , gamma-aminobutyrate , aspartate and glycine , were released from rat brain slices on incubation with protoveratrine ( especially in a Ca ( 2 + ) - deficient medium ) or with ouabain or in the absence of glucose .
	manualset3
220963	3	420611	7	NULL	NULL	0	NULL	gamma-aminobutyrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino acids , particularly glutamate , gamma-aminobutyrate , aspartate and glycine , were released from rat brain slices on incubation with protoveratrine ( especially in a Ca ( 2 + ) - deficient medium ) or with ouabain or in the absence of glucose .
	manualset3
220964	4	420611	7	NULL	NULL	0	NULL	aspartate 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino acids , particularly glutamate , gamma-aminobutyrate , aspartate and glycine , were released from rat brain slices on incubation with protoveratrine ( especially in a Ca ( 2 + ) - deficient medium ) or with ouabain or in the absence of glucose .
	manualset3
220965	5	420611	7	NULL	NULL	0	NULL	glycine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino acids , particularly glutamate , gamma-aminobutyrate , aspartate and glycine , were released from rat brain slices on incubation with protoveratrine ( especially in a Ca ( 2 + ) - deficient medium ) or with ouabain or in the absence of glucose .
	manualset3
220966	6	420611	7	NULL	NULL	0	NULL	rat brain slices	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino acids , particularly glutamate , gamma-aminobutyrate , aspartate and glycine , were released from rat brain slices on incubation with protoveratrine ( especially in a Ca ( 2 + ) - deficient medium ) or with ouabain or in the absence of glucose .
	manualset3
220967	7	420611	7	NULL	NULL	0	NULL	incubation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino acids , particularly glutamate , gamma-aminobutyrate , aspartate and glycine , were released from rat brain slices on incubation with protoveratrine ( especially in a Ca ( 2 + ) - deficient medium ) or with ouabain or in the absence of glucose .
	manualset3
220968	8	420611	7	NULL	NULL	0	NULL	protoveratrine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino acids , particularly glutamate , gamma-aminobutyrate , aspartate and glycine , were released from rat brain slices on incubation with protoveratrine ( especially in a Ca ( 2 + ) - deficient medium ) or with ouabain or in the absence of glucose .
	manualset3
220969	9	420611	7	NULL	NULL	0	NULL	Ca ( 2 + ) - deficient medium	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino acids , particularly glutamate , gamma-aminobutyrate , aspartate and glycine , were released from rat brain slices on incubation with protoveratrine ( especially in a Ca ( 2 + ) - deficient medium ) or with ouabain or in the absence of glucose .
	manualset3
220970	10	420611	7	NULL	NULL	0	NULL	ouabain 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino acids , particularly glutamate , gamma-aminobutyrate , aspartate and glycine , were released from rat brain slices on incubation with protoveratrine ( especially in a Ca ( 2 + ) - deficient medium ) or with ouabain or in the absence of glucose .
	manualset3
220971	11	420611	7	NULL	NULL	0	NULL	absence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino acids , particularly glutamate , gamma-aminobutyrate , aspartate and glycine , were released from rat brain slices on incubation with protoveratrine ( especially in a Ca ( 2 + ) - deficient medium ) or with ouabain or in the absence of glucose .
	manualset3
220972	12	420611	7	NULL	NULL	0	NULL	glucose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Amino acids , particularly glutamate , gamma-aminobutyrate , aspartate and glycine , were released from rat brain slices on incubation with protoveratrine ( especially in a Ca ( 2 + ) - deficient medium ) or with ouabain or in the absence of glucose .
	manualset3
220973	1	420612	7	NULL	NULL	0	NULL	Ambulatory laparoscopic cholecystectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Ambulatory laparoscopic cholecystectomy is as effective as hospitalization and from a social perspective less expensive : a randomized study ) .
	manualset3
220974	2	420612	7	NULL	NULL	0	NULL	hospitalization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Ambulatory laparoscopic cholecystectomy is as effective as hospitalization and from a social perspective less expensive : a randomized study ) .
	manualset3
220975	3	420612	7	NULL	NULL	0	NULL	social perspective	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Ambulatory laparoscopic cholecystectomy is as effective as hospitalization and from a social perspective less expensive : a randomized study ) .
	manualset3
220976	4	420612	7	NULL	NULL	0	NULL	randomized study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Ambulatory laparoscopic cholecystectomy is as effective as hospitalization and from a social perspective less expensive : a randomized study ) .
	manualset3
220977	1	420613	7	NULL	NULL	0	NULL	degree	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the degree nor the direction of displacement prevented union , which occurred in all 13 .
	manualset3
220978	2	420613	7	NULL	NULL	0	NULL	direction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the degree nor the direction of displacement prevented union , which occurred in all 13 .
	manualset3
220979	3	420613	7	NULL	NULL	0	NULL	displacement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the degree nor the direction of displacement prevented union , which occurred in all 13 .
	manualset3
220980	4	420613	7	NULL	NULL	0	NULL	union	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the degree nor the direction of displacement prevented union , which occurred in all 13 .
	manualset3
220981	5	420613	7	NULL	NULL	0	NULL	13	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Neither the degree nor the direction of displacement prevented union , which occurred in all 13 .
	manualset3
220982	1	420614	7	NULL	NULL	0	NULL	Modified Rubner 's test	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Modified Rubner 's test : diagnosis of secondary lactose intolerance diarrhea .
	manualset3
220983	2	420614	7	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Modified Rubner 's test : diagnosis of secondary lactose intolerance diarrhea .
	manualset3
220984	3	420614	7	NULL	NULL	0	NULL	secondary lactose intolerance diarrhea	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Modified Rubner 's test : diagnosis of secondary lactose intolerance diarrhea .
	manualset3
220985	1	420615	7	NULL	NULL	0	NULL	IL-15 cultured T cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , IL-15 cultured T cells showed an increase in cytolytic effector molecules .
	manualset3
220986	3	420615	7	NULL	NULL	NULL	NULL	cytolytic effector molecules	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Additionally , IL-15 cultured T cells showed an increase in cytolytic effector molecules .
	manualset3
220987	2	420615	7	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , IL-15 cultured T cells showed an increase in cytolytic effector molecules .
	manualset3
220988	1	420616	7	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , this problem was addressed by transfecting primary cultures of human pulp cells with an SV40-adenovirus construct .
	manualset3
220989	2	420616	7	NULL	NULL	0	NULL	problem	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , this problem was addressed by transfecting primary cultures of human pulp cells with an SV40-adenovirus construct .
	manualset3
220990	3	420616	7	NULL	NULL	0	NULL	primary cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , this problem was addressed by transfecting primary cultures of human pulp cells with an SV40-adenovirus construct .
	manualset3
220991	4	420616	7	NULL	NULL	0	NULL	human pulp cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , this problem was addressed by transfecting primary cultures of human pulp cells with an SV40-adenovirus construct .
	manualset3
220992	5	420616	7	NULL	NULL	0	NULL	SV40-adenovirus construct	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , this problem was addressed by transfecting primary cultures of human pulp cells with an SV40-adenovirus construct .
	manualset3
220993	1	420617	7	NULL	NULL	0	NULL	Temozolomide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Temozolomide is a prodrug that undergoes spontaneous chemical degradation at physiologic pH to form the highly reactive alkylating agent , methyl-triazenyl imidazole carboxamide ( MTIC ) .
	manualset3
220994	2	420617	7	NULL	NULL	0	NULL	prodrug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Temozolomide is a prodrug that undergoes spontaneous chemical degradation at physiologic pH to form the highly reactive alkylating agent , methyl-triazenyl imidazole carboxamide ( MTIC ) .
	manualset3
220995	3	420617	7	NULL	NULL	0	NULL	spontaneous chemical degradation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Temozolomide is a prodrug that undergoes spontaneous chemical degradation at physiologic pH to form the highly reactive alkylating agent , methyl-triazenyl imidazole carboxamide ( MTIC ) .
	manualset3
220996	4	420617	7	NULL	NULL	0	NULL	physiologic pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Temozolomide is a prodrug that undergoes spontaneous chemical degradation at physiologic pH to form the highly reactive alkylating agent , methyl-triazenyl imidazole carboxamide ( MTIC ) .
	manualset3
220997	5	420617	7	NULL	NULL	0	NULL	 highly reactive alkylating agent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Temozolomide is a prodrug that undergoes spontaneous chemical degradation at physiologic pH to form the highly reactive alkylating agent , methyl-triazenyl imidazole carboxamide ( MTIC ) .
	manualset3
220998	6	420617	7	NULL	NULL	0	NULL	methyl-triazenyl imidazole carboxamide ( MTIC ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Temozolomide is a prodrug that undergoes spontaneous chemical degradation at physiologic pH to form the highly reactive alkylating agent , methyl-triazenyl imidazole carboxamide ( MTIC ) .
	manualset3
220999	1	420618	7	NULL	NULL	0	NULL	calculations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These calculations require hours to a day on a commodity computer .
	manualset3
221000	2	420618	7	NULL	NULL	0	NULL	hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	These calculations require hours to a day on a commodity computer .
	manualset3
221001	3	420618	7	NULL	NULL	0	NULL	 day 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	These calculations require hours to a day on a commodity computer .
	manualset3
221002	4	420618	7	NULL	NULL	0	NULL	commodity computer	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	These calculations require hours to a day on a commodity computer .
	manualset3
221003	1	420619	7	NULL	NULL	0	NULL	 movable wires	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	This was tested by implanting movable and stationary wires in the medullary canal of the rabbit femora or tibiae .
	manualset3
221004	2	420619	7	NULL	NULL	0	NULL	stationary wires	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	This was tested by implanting movable and stationary wires in the medullary canal of the rabbit femora or tibiae .
	manualset3
221005	3	420619	7	NULL	NULL	0	NULL	medullary canal	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This was tested by implanting movable and stationary wires in the medullary canal of the rabbit femora or tibiae .
	manualset3
221006	4	420619	7	NULL	NULL	0	NULL	 rabbit femora	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This was tested by implanting movable and stationary wires in the medullary canal of the rabbit femora or tibiae .
	manualset3
221007	5	420619	7	NULL	NULL	0	NULL	tibiae	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This was tested by implanting movable and stationary wires in the medullary canal of the rabbit femora or tibiae .
	manualset3
221008	1	420620	7	NULL	NULL	NULL	NULL	siRNA vector - transfected Hela cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The siRNA vector - transfected Hela cells and SSOP-9607 cells revealed marked inhibition of stathmin expression and a dramatic growth inhibition comparing with ECV304 cells , parental-vector transfected cells and untransfected cells .
	manualset3
221009	2	420620	7	NULL	NULL	0	NULL	 SSOP-9607 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The siRNA vector - transfected Hela cells and SSOP-9607 cells revealed marked inhibition of stathmin expression and a dramatic growth inhibition comparing with ECV304 cells , parental-vector transfected cells and untransfected cells .
	manualset3
221010	3	420620	7	NULL	NULL	0	NULL	marked inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The siRNA vector - transfected Hela cells and SSOP-9607 cells revealed marked inhibition of stathmin expression and a dramatic growth inhibition comparing with ECV304 cells , parental-vector transfected cells and untransfected cells .
	manualset3
221011	4	420620	7	NULL	NULL	0	NULL	stathmin expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The siRNA vector - transfected Hela cells and SSOP-9607 cells revealed marked inhibition of stathmin expression and a dramatic growth inhibition comparing with ECV304 cells , parental-vector transfected cells and untransfected cells .
	manualset3
221012	5	420620	7	NULL	NULL	0	NULL	dramatic growth inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The siRNA vector - transfected Hela cells and SSOP-9607 cells revealed marked inhibition of stathmin expression and a dramatic growth inhibition comparing with ECV304 cells , parental-vector transfected cells and untransfected cells .
	manualset3
221013	6	420620	7	NULL	NULL	0	NULL	ECV304 cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The siRNA vector - transfected Hela cells and SSOP-9607 cells revealed marked inhibition of stathmin expression and a dramatic growth inhibition comparing with ECV304 cells , parental-vector transfected cells and untransfected cells .
	manualset3
221014	7	420620	7	NULL	NULL	0	NULL	parental-vector transfected cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The siRNA vector - transfected Hela cells and SSOP-9607 cells revealed marked inhibition of stathmin expression and a dramatic growth inhibition comparing with ECV304 cells , parental-vector transfected cells and untransfected cells .
	manualset3
221015	8	420620	7	NULL	NULL	0	NULL	untransfected cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The siRNA vector - transfected Hela cells and SSOP-9607 cells revealed marked inhibition of stathmin expression and a dramatic growth inhibition comparing with ECV304 cells , parental-vector transfected cells and untransfected cells .
	manualset3
221016	1	420621	7	NULL	NULL	0	NULL	 cytosol	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cytosol of intact rat ovary a significant fraction of the total binding sites was found to be occupied , presumably by the endogenous estrogen .
	manualset3
221017	2	420621	7	NULL	NULL	0	NULL	intact rat ovary 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cytosol of intact rat ovary a significant fraction of the total binding sites was found to be occupied , presumably by the endogenous estrogen .
	manualset3
221018	3	420621	7	NULL	NULL	NULL	NULL	significant fraction 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In the cytosol of intact rat ovary a significant fraction of the total binding sites was found to be occupied , presumably by the endogenous estrogen .
	manualset3
221019	4	420621	7	NULL	NULL	0	NULL	 total binding sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cytosol of intact rat ovary a significant fraction of the total binding sites was found to be occupied , presumably by the endogenous estrogen .
	manualset3
221020	5	420621	7	NULL	NULL	0	NULL	endogenous estrogen	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cytosol of intact rat ovary a significant fraction of the total binding sites was found to be occupied , presumably by the endogenous estrogen .
	manualset3
221021	1	420622	7	NULL	NULL	0	NULL	 initial concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With increasing initial concentration of Cr ( VI ) , the adsorption rate constant decreased while the maximum adsorption capacity increased .
	manualset3
221022	2	420622	7	NULL	NULL	0	NULL	Cr ( VI )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	With increasing initial concentration of Cr ( VI ) , the adsorption rate constant decreased while the maximum adsorption capacity increased .
	manualset3
221023	3	420622	7	NULL	NULL	0	NULL	adsorption rate constant	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With increasing initial concentration of Cr ( VI ) , the adsorption rate constant decreased while the maximum adsorption capacity increased .
	manualset3
221024	4	420622	7	NULL	NULL	0	NULL	maximum adsorption capacity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With increasing initial concentration of Cr ( VI ) , the adsorption rate constant decreased while the maximum adsorption capacity increased .
	manualset3
221025	1	420623	7	NULL	NULL	0	NULL	proper staging system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A more proper staging system might also be needed to analyze clinical studies .
	manualset3
221026	2	420623	7	NULL	NULL	0	NULL	clinical studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A more proper staging system might also be needed to analyze clinical studies .
	manualset3
221027	1	420624	7	NULL	NULL	0	NULL	Subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects with asbestosis had a moderate neutrophilic alveolitis ( 7.8 + / - 5 % ) compared with the other groups ( p less than 0.001 ) that was correlated with the presence of crackles ( p = 0.03 ) and PaO2 ( p less than 0.05 ) and AaPO2 at rest ( p less than 0.05 ) values .
	manualset3
221028	2	420624	7	NULL	NULL	0	NULL	asbestosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects with asbestosis had a moderate neutrophilic alveolitis ( 7.8 + / - 5 % ) compared with the other groups ( p less than 0.001 ) that was correlated with the presence of crackles ( p = 0.03 ) and PaO2 ( p less than 0.05 ) and AaPO2 at rest ( p less than 0.05 ) values .
	manualset3
221029	3	420624	7	NULL	NULL	0	NULL	moderate neutrophilic alveolitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects with asbestosis had a moderate neutrophilic alveolitis ( 7.8 + / - 5 % ) compared with the other groups ( p less than 0.001 ) that was correlated with the presence of crackles ( p = 0.03 ) and PaO2 ( p less than 0.05 ) and AaPO2 at rest ( p less than 0.05 ) values .
	manualset3
221030	4	420624	7	NULL	NULL	0	NULL	7.8 + / - 5 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects with asbestosis had a moderate neutrophilic alveolitis ( 7.8 + / - 5 % ) compared with the other groups ( p less than 0.001 ) that was correlated with the presence of crackles ( p = 0.03 ) and PaO2 ( p less than 0.05 ) and AaPO2 at rest ( p less than 0.05 ) values .
	manualset3
221031	5	420624	7	NULL	NULL	0	NULL	other groups 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects with asbestosis had a moderate neutrophilic alveolitis ( 7.8 + / - 5 % ) compared with the other groups ( p less than 0.001 ) that was correlated with the presence of crackles ( p = 0.03 ) and PaO2 ( p less than 0.05 ) and AaPO2 at rest ( p less than 0.05 ) values .
	manualset3
221032	6	420624	7	NULL	NULL	0	NULL	p less than 0.001	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects with asbestosis had a moderate neutrophilic alveolitis ( 7.8 + / - 5 % ) compared with the other groups ( p less than 0.001 ) that was correlated with the presence of crackles ( p = 0.03 ) and PaO2 ( p less than 0.05 ) and AaPO2 at rest ( p less than 0.05 ) values .
	manualset3
221033	7	420624	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects with asbestosis had a moderate neutrophilic alveolitis ( 7.8 + / - 5 % ) compared with the other groups ( p less than 0.001 ) that was correlated with the presence of crackles ( p = 0.03 ) and PaO2 ( p less than 0.05 ) and AaPO2 at rest ( p less than 0.05 ) values .
	manualset3
221034	8	420624	7	NULL	NULL	0	NULL	crackles	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects with asbestosis had a moderate neutrophilic alveolitis ( 7.8 + / - 5 % ) compared with the other groups ( p less than 0.001 ) that was correlated with the presence of crackles ( p = 0.03 ) and PaO2 ( p less than 0.05 ) and AaPO2 at rest ( p less than 0.05 ) values .
	manualset3
221035	9	420624	7	NULL	NULL	0	NULL	p = 0.03 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects with asbestosis had a moderate neutrophilic alveolitis ( 7.8 + / - 5 % ) compared with the other groups ( p less than 0.001 ) that was correlated with the presence of crackles ( p = 0.03 ) and PaO2 ( p less than 0.05 ) and AaPO2 at rest ( p less than 0.05 ) values .
	manualset3
221036	10	420624	7	NULL	NULL	0	NULL	PaO2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects with asbestosis had a moderate neutrophilic alveolitis ( 7.8 + / - 5 % ) compared with the other groups ( p less than 0.001 ) that was correlated with the presence of crackles ( p = 0.03 ) and PaO2 ( p less than 0.05 ) and AaPO2 at rest ( p less than 0.05 ) values .
	manualset3
221037	11	420624	7	NULL	NULL	0	NULL	p less than 0.05	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects with asbestosis had a moderate neutrophilic alveolitis ( 7.8 + / - 5 % ) compared with the other groups ( p less than 0.001 ) that was correlated with the presence of crackles ( p = 0.03 ) and PaO2 ( p less than 0.05 ) and AaPO2 at rest ( p less than 0.05 ) values .
	manualset3
221038	12	420624	7	NULL	NULL	0	NULL	AaPO2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects with asbestosis had a moderate neutrophilic alveolitis ( 7.8 + / - 5 % ) compared with the other groups ( p less than 0.001 ) that was correlated with the presence of crackles ( p = 0.03 ) and PaO2 ( p less than 0.05 ) and AaPO2 at rest ( p less than 0.05 ) values .
	manualset3
221039	13	420624	7	NULL	NULL	0	NULL	rest values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects with asbestosis had a moderate neutrophilic alveolitis ( 7.8 + / - 5 % ) compared with the other groups ( p less than 0.001 ) that was correlated with the presence of crackles ( p = 0.03 ) and PaO2 ( p less than 0.05 ) and AaPO2 at rest ( p less than 0.05 ) values .
	manualset3
221040	14	420624	7	NULL	NULL	0	NULL	p less than 0.05	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects with asbestosis had a moderate neutrophilic alveolitis ( 7.8 + / - 5 % ) compared with the other groups ( p less than 0.001 ) that was correlated with the presence of crackles ( p = 0.03 ) and PaO2 ( p less than 0.05 ) and AaPO2 at rest ( p less than 0.05 ) values .
	manualset3
221041	1	420625	7	NULL	NULL	0	NULL	 authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors came to conclusion that months of seasonal pickup in Orenburg region are September - December , January of next year ; in Totskiy region -- November - February .
	manualset3
221042	2	420625	7	NULL	NULL	0	NULL	 conclusion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors came to conclusion that months of seasonal pickup in Orenburg region are September - December , January of next year ; in Totskiy region -- November - February .
	manualset3
221043	3	420625	7	NULL	NULL	0	NULL	months 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors came to conclusion that months of seasonal pickup in Orenburg region are September - December , January of next year ; in Totskiy region -- November - February .
	manualset3
221044	4	420625	7	NULL	NULL	0	NULL	seasonal pickup	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors came to conclusion that months of seasonal pickup in Orenburg region are September - December , January of next year ; in Totskiy region -- November - February .
	manualset3
221045	5	420625	7	NULL	NULL	0	NULL	Orenburg region 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors came to conclusion that months of seasonal pickup in Orenburg region are September - December , January of next year ; in Totskiy region -- November - February .
	manualset3
221046	6	420625	7	NULL	NULL	0	NULL	September - December	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors came to conclusion that months of seasonal pickup in Orenburg region are September - December , January of next year ; in Totskiy region -- November - February .
	manualset3
221047	7	420625	7	NULL	NULL	0	NULL	January	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors came to conclusion that months of seasonal pickup in Orenburg region are September - December , January of next year ; in Totskiy region -- November - February .
	manualset3
221048	8	420625	7	NULL	NULL	NULL	NULL	next year	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The authors came to conclusion that months of seasonal pickup in Orenburg region are September - December , January of next year ; in Totskiy region -- November - February .
	manualset3
221049	9	420625	7	NULL	NULL	0	NULL	Totskiy region	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors came to conclusion that months of seasonal pickup in Orenburg region are September - December , January of next year ; in Totskiy region -- November - February .
	manualset3
221050	10	420625	7	NULL	NULL	0	NULL	November - February	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors came to conclusion that months of seasonal pickup in Orenburg region are September - December , January of next year ; in Totskiy region -- November - February .
	manualset3
221051	1	420626	7	NULL	NULL	0	NULL	unusual source	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	An unusual source for postmortem findings of methyl ethyl ketone and methanol in two homicide victims .
	manualset3
221052	2	420626	7	NULL	NULL	0	NULL	postmortem findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An unusual source for postmortem findings of methyl ethyl ketone and methanol in two homicide victims .
	manualset3
221053	3	420626	7	NULL	NULL	0	NULL	methyl ethyl ketone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An unusual source for postmortem findings of methyl ethyl ketone and methanol in two homicide victims .
	manualset3
221054	4	420626	7	NULL	NULL	0	NULL	methanol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An unusual source for postmortem findings of methyl ethyl ketone and methanol in two homicide victims .
	manualset3
221055	5	420626	7	NULL	NULL	0	NULL	two homicide victims	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	An unusual source for postmortem findings of methyl ethyl ketone and methanol in two homicide victims .
	manualset3
221056	1	420627	7	NULL	NULL	0	NULL	Activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of HIV in human skin by ultraviolet B radiation and its inhibition by NFkappaB blocking agents .
	manualset3
221057	2	420627	7	NULL	NULL	0	NULL	HIV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of HIV in human skin by ultraviolet B radiation and its inhibition by NFkappaB blocking agents .
	manualset3
221058	3	420627	7	NULL	NULL	0	NULL	human skin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of HIV in human skin by ultraviolet B radiation and its inhibition by NFkappaB blocking agents .
	manualset3
221059	4	420627	7	NULL	NULL	0	NULL	ultraviolet B radiation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of HIV in human skin by ultraviolet B radiation and its inhibition by NFkappaB blocking agents .
	manualset3
221060	5	420627	7	NULL	NULL	0	NULL	inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of HIV in human skin by ultraviolet B radiation and its inhibition by NFkappaB blocking agents .
	manualset3
221061	6	420627	7	NULL	NULL	0	NULL	NFkappaB blocking agents 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Activation of HIV in human skin by ultraviolet B radiation and its inhibition by NFkappaB blocking agents .
	manualset3
221062	1	420628	7	NULL	NULL	0	NULL	1938	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1938 , P. K. Wrigley , owner of the Chicago Cubs , hired him to help improve the team 's performance .
	manualset3
221063	2	420628	7	NULL	NULL	0	NULL	P. K. Wrigley	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1938 , P. K. Wrigley , owner of the Chicago Cubs , hired him to help improve the team 's performance .
	manualset3
221064	3	420628	7	NULL	NULL	0	NULL	owner	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1938 , P. K. Wrigley , owner of the Chicago Cubs , hired him to help improve the team 's performance .
	manualset3
221065	4	420628	7	NULL	NULL	0	NULL	Chicago Cubs	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1938 , P. K. Wrigley , owner of the Chicago Cubs , hired him to help improve the team 's performance .
	manualset3
221066	5	420628	7	NULL	NULL	0	NULL	team 's performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1938 , P. K. Wrigley , owner of the Chicago Cubs , hired him to help improve the team 's performance .
	manualset3
221067	1	420629	7	NULL	NULL	0	NULL	expression profiles	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We compared expression profiles of the cells at days 3 , 15 , and 27 of incubation in media containing either a combination of 0.1 microM dexamethasone , 0.05 mM ascorbic acid-2-phosphate , and 10 mM beta-glycerophosphate , dexamethasone only , ascorbic acid-2-phosphate plus beta-glycerophosphate , or medium without any of these osteogenic supplements .
	manualset3
221068	2	420629	7	NULL	NULL	NULL	NULL	cells	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We compared expression profiles of the cells at days 3 , 15 , and 27 of incubation in media containing either a combination of 0.1 microM dexamethasone , 0.05 mM ascorbic acid-2-phosphate , and 10 mM beta-glycerophosphate , dexamethasone only , ascorbic acid-2-phosphate plus beta-glycerophosphate , or medium without any of these osteogenic supplements .
	manualset3
221069	3	420629	7	NULL	NULL	0	NULL	days 3	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	We compared expression profiles of the cells at days 3 , 15 , and 27 of incubation in media containing either a combination of 0.1 microM dexamethasone , 0.05 mM ascorbic acid-2-phosphate , and 10 mM beta-glycerophosphate , dexamethasone only , ascorbic acid-2-phosphate plus beta-glycerophosphate , or medium without any of these osteogenic supplements .
	manualset3
221070	4	420629	7	NULL	NULL	0	NULL	days 15	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	We compared expression profiles of the cells at days 3 , 15 , and 27 of incubation in media containing either a combination of 0.1 microM dexamethasone , 0.05 mM ascorbic acid-2-phosphate , and 10 mM beta-glycerophosphate , dexamethasone only , ascorbic acid-2-phosphate plus beta-glycerophosphate , or medium without any of these osteogenic supplements .
	manualset3
221071	5	420629	7	NULL	NULL	0	NULL	days 27	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	We compared expression profiles of the cells at days 3 , 15 , and 27 of incubation in media containing either a combination of 0.1 microM dexamethasone , 0.05 mM ascorbic acid-2-phosphate , and 10 mM beta-glycerophosphate , dexamethasone only , ascorbic acid-2-phosphate plus beta-glycerophosphate , or medium without any of these osteogenic supplements .
	manualset3
221072	6	420629	7	NULL	NULL	0	NULL	incubation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We compared expression profiles of the cells at days 3 , 15 , and 27 of incubation in media containing either a combination of 0.1 microM dexamethasone , 0.05 mM ascorbic acid-2-phosphate , and 10 mM beta-glycerophosphate , dexamethasone only , ascorbic acid-2-phosphate plus beta-glycerophosphate , or medium without any of these osteogenic supplements .
	manualset3
221073	7	420629	7	NULL	NULL	0	NULL	media 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We compared expression profiles of the cells at days 3 , 15 , and 27 of incubation in media containing either a combination of 0.1 microM dexamethasone , 0.05 mM ascorbic acid-2-phosphate , and 10 mM beta-glycerophosphate , dexamethasone only , ascorbic acid-2-phosphate plus beta-glycerophosphate , or medium without any of these osteogenic supplements .
	manualset3
221074	8	420629	7	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We compared expression profiles of the cells at days 3 , 15 , and 27 of incubation in media containing either a combination of 0.1 microM dexamethasone , 0.05 mM ascorbic acid-2-phosphate , and 10 mM beta-glycerophosphate , dexamethasone only , ascorbic acid-2-phosphate plus beta-glycerophosphate , or medium without any of these osteogenic supplements .
	manualset3
221075	9	420629	7	NULL	NULL	0	NULL	0.1 microM dexamethasone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We compared expression profiles of the cells at days 3 , 15 , and 27 of incubation in media containing either a combination of 0.1 microM dexamethasone , 0.05 mM ascorbic acid-2-phosphate , and 10 mM beta-glycerophosphate , dexamethasone only , ascorbic acid-2-phosphate plus beta-glycerophosphate , or medium without any of these osteogenic supplements .
	manualset3
221076	10	420629	7	NULL	NULL	0	NULL	0.05 mM ascorbic acid-2-phosphate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We compared expression profiles of the cells at days 3 , 15 , and 27 of incubation in media containing either a combination of 0.1 microM dexamethasone , 0.05 mM ascorbic acid-2-phosphate , and 10 mM beta-glycerophosphate , dexamethasone only , ascorbic acid-2-phosphate plus beta-glycerophosphate , or medium without any of these osteogenic supplements .
	manualset3
221077	11	420629	7	NULL	NULL	0	NULL	10 mM beta-glycerophosphate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We compared expression profiles of the cells at days 3 , 15 , and 27 of incubation in media containing either a combination of 0.1 microM dexamethasone , 0.05 mM ascorbic acid-2-phosphate , and 10 mM beta-glycerophosphate , dexamethasone only , ascorbic acid-2-phosphate plus beta-glycerophosphate , or medium without any of these osteogenic supplements .
	manualset3
221078	12	420629	7	NULL	NULL	0	NULL	dexamethasone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We compared expression profiles of the cells at days 3 , 15 , and 27 of incubation in media containing either a combination of 0.1 microM dexamethasone , 0.05 mM ascorbic acid-2-phosphate , and 10 mM beta-glycerophosphate , dexamethasone only , ascorbic acid-2-phosphate plus beta-glycerophosphate , or medium without any of these osteogenic supplements .
	manualset3
221079	13	420629	7	NULL	NULL	0	NULL	ascorbic acid-2-phosphate plus beta-glycerophosphate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We compared expression profiles of the cells at days 3 , 15 , and 27 of incubation in media containing either a combination of 0.1 microM dexamethasone , 0.05 mM ascorbic acid-2-phosphate , and 10 mM beta-glycerophosphate , dexamethasone only , ascorbic acid-2-phosphate plus beta-glycerophosphate , or medium without any of these osteogenic supplements .
	manualset3
221080	14	420629	7	NULL	NULL	0	NULL	medium	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We compared expression profiles of the cells at days 3 , 15 , and 27 of incubation in media containing either a combination of 0.1 microM dexamethasone , 0.05 mM ascorbic acid-2-phosphate , and 10 mM beta-glycerophosphate , dexamethasone only , ascorbic acid-2-phosphate plus beta-glycerophosphate , or medium without any of these osteogenic supplements .
	manualset3
221081	15	420629	7	NULL	NULL	0	NULL	osteogenic supplements	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We compared expression profiles of the cells at days 3 , 15 , and 27 of incubation in media containing either a combination of 0.1 microM dexamethasone , 0.05 mM ascorbic acid-2-phosphate , and 10 mM beta-glycerophosphate , dexamethasone only , ascorbic acid-2-phosphate plus beta-glycerophosphate , or medium without any of these osteogenic supplements .
	manualset3
221082	1	420630	7	NULL	NULL	0	NULL	end of the delay	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	At the end of the delay , subjects were required to begin movement rapidly .
	manualset3
221083	2	420630	7	NULL	NULL	0	NULL	subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	At the end of the delay , subjects were required to begin movement rapidly .
	manualset3
221084	3	420630	7	NULL	NULL	0	NULL	movement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	At the end of the delay , subjects were required to begin movement rapidly .
	manualset3
221086	1	420631	7	NULL	NULL	0	NULL	conclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , OPG concentrations are increased in patients with RA and are associated with inflammation .
	manualset3
221087	2	420631	7	NULL	NULL	0	NULL	OPG concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , OPG concentrations are increased in patients with RA and are associated with inflammation .
	manualset3
221088	3	420631	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , OPG concentrations are increased in patients with RA and are associated with inflammation .
	manualset3
221089	4	420631	7	NULL	NULL	0	NULL	RA	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , OPG concentrations are increased in patients with RA and are associated with inflammation .
	manualset3
221090	5	420631	7	NULL	NULL	0	NULL	inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , OPG concentrations are increased in patients with RA and are associated with inflammation .
	manualset3
221091	1	420632	7	NULL	NULL	0	NULL	four frozen gel pack configuration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A modified four frozen gel pack configuration was suitable for summer transit .
	manualset3
221092	2	420632	7	NULL	NULL	0	NULL	summer transit	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A modified four frozen gel pack configuration was suitable for summer transit .
	manualset3
221093	1	420633	7	NULL	NULL	0	NULL	increased lipid damage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased lipid damage observed in nIDC correlates with estrogen receptor exposure in IDC ( R ( 2 ) = 0.89 ) .
	manualset3
221180	2	420633	7	NULL	NULL	0	NULL	nIDC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased lipid damage observed in nIDC correlates with estrogen receptor exposure in IDC ( R ( 2 ) = 0.89 ) .
	manualset3
221181	3	420633	7	NULL	NULL	0	NULL	estrogen receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased lipid damage observed in nIDC correlates with estrogen receptor exposure in IDC ( R ( 2 ) = 0.89 ) .
	manualset3
221182	4	420633	7	NULL	NULL	0	NULL	 IDC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased lipid damage observed in nIDC correlates with estrogen receptor exposure in IDC ( R ( 2 ) = 0.89 ) .
	manualset3
221183	5	420633	7	NULL	NULL	0	NULL	R ( 2 ) = 0.89	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased lipid damage observed in nIDC correlates with estrogen receptor exposure in IDC ( R ( 2 ) = 0.89 ) .
	manualset3
221184	1	420634	7	NULL	NULL	0	NULL	 injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After the injection ( 30 micrograms microliters-1 ) the monkeys tended to use the contralateral hand , and the ipsilateral hand showed a posture of dropped wrist and fingers , as if the radial nerve were paralysed .
	manualset3
221185	2	420634	7	NULL	NULL	0	NULL	30 micrograms microliters-1	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	After the injection ( 30 micrograms microliters-1 ) the monkeys tended to use the contralateral hand , and the ipsilateral hand showed a posture of dropped wrist and fingers , as if the radial nerve were paralysed .
	manualset3
221186	3	420634	7	NULL	NULL	0	NULL	monkeys	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	After the injection ( 30 micrograms microliters-1 ) the monkeys tended to use the contralateral hand , and the ipsilateral hand showed a posture of dropped wrist and fingers , as if the radial nerve were paralysed .
	manualset3
221187	4	420634	7	NULL	NULL	0	NULL	contralateral hand	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After the injection ( 30 micrograms microliters-1 ) the monkeys tended to use the contralateral hand , and the ipsilateral hand showed a posture of dropped wrist and fingers , as if the radial nerve were paralysed .
	manualset3
221188	5	420634	7	NULL	NULL	0	NULL	ipsilateral hand	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After the injection ( 30 micrograms microliters-1 ) the monkeys tended to use the contralateral hand , and the ipsilateral hand showed a posture of dropped wrist and fingers , as if the radial nerve were paralysed .
	manualset3
221189	6	420634	7	NULL	NULL	0	NULL	posture	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After the injection ( 30 micrograms microliters-1 ) the monkeys tended to use the contralateral hand , and the ipsilateral hand showed a posture of dropped wrist and fingers , as if the radial nerve were paralysed .
	manualset3
221190	7	420634	7	NULL	NULL	0	NULL	dropped wrist	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After the injection ( 30 micrograms microliters-1 ) the monkeys tended to use the contralateral hand , and the ipsilateral hand showed a posture of dropped wrist and fingers , as if the radial nerve were paralysed .
	manualset3
221191	8	420634	7	NULL	NULL	0	NULL	 fingers 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After the injection ( 30 micrograms microliters-1 ) the monkeys tended to use the contralateral hand , and the ipsilateral hand showed a posture of dropped wrist and fingers , as if the radial nerve were paralysed .
	manualset3
221192	9	420634	7	NULL	NULL	0	NULL	 radial nerve	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After the injection ( 30 micrograms microliters-1 ) the monkeys tended to use the contralateral hand , and the ipsilateral hand showed a posture of dropped wrist and fingers , as if the radial nerve were paralysed .
	manualset3
221196	1	420635	7	NULL	NULL	0	NULL	COX-2 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	COX-2 expression increases during progression from a normal to cancerous state .
	manualset3
221198	2	420635	7	NULL	NULL	0	NULL	progression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	COX-2 expression increases during progression from a normal to cancerous state .
	manualset3
221201	3	420635	7	NULL	NULL	0	NULL	normal	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	COX-2 expression increases during progression from a normal to cancerous state .
	manualset3
221202	4	420635	7	NULL	NULL	0	NULL	 cancerous state	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	COX-2 expression increases during progression from a normal to cancerous state .
	manualset3
221203	1	420636	7	NULL	NULL	0	NULL	Ammoniation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ammoniation of kenaf tops prior to dehydration .
	manualset3
221204	2	420636	7	NULL	NULL	0	NULL	kenaf tops	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ammoniation of kenaf tops prior to dehydration .
	manualset3
221205	3	420636	7	NULL	NULL	0	NULL	dehydration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ammoniation of kenaf tops prior to dehydration .
	manualset3
221206	1	420637	7	NULL	NULL	0	NULL	Significant effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant effect of ABO blood groups on the aggregation of red cells in patients with diabetes mellitus .
	manualset3
221207	2	420637	7	NULL	NULL	0	NULL	ABO blood groups	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant effect of ABO blood groups on the aggregation of red cells in patients with diabetes mellitus .
	manualset3
221208	3	420637	7	NULL	NULL	0	NULL	aggregation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant effect of ABO blood groups on the aggregation of red cells in patients with diabetes mellitus .
	manualset3
221209	4	420637	7	NULL	NULL	0	NULL	red cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant effect of ABO blood groups on the aggregation of red cells in patients with diabetes mellitus .
	manualset3
221210	5	420637	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant effect of ABO blood groups on the aggregation of red cells in patients with diabetes mellitus .
	manualset3
221211	6	420637	7	NULL	NULL	0	NULL	diabetes mellitus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Significant effect of ABO blood groups on the aggregation of red cells in patients with diabetes mellitus .
	manualset3
221212	1	420638	7	NULL	NULL	0	NULL	6 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In only 6 patients ( 10 % ) was the anterior leaflet alone responsible for SAM .
	manualset3
221221	2	420638	7	NULL	NULL	0	NULL	10 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In only 6 patients ( 10 % ) was the anterior leaflet alone responsible for SAM .
	manualset3
221243	3	420638	7	NULL	NULL	0	NULL	anterior leaflet 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In only 6 patients ( 10 % ) was the anterior leaflet alone responsible for SAM .
	manualset3
221244	4	420638	7	NULL	NULL	0	NULL	SAM	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In only 6 patients ( 10 % ) was the anterior leaflet alone responsible for SAM .
	manualset3
221245	1	420639	7	NULL	NULL	0	NULL	1996	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1996 , 19 isolates of serotype 6B Streptococcus pneumoniae with a unique resistance pattern were found in carriers attending daycare centres in Patras , Southwestern Greece .
	manualset3
221246	2	420639	7	NULL	NULL	0	NULL	19 isolates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1996 , 19 isolates of serotype 6B Streptococcus pneumoniae with a unique resistance pattern were found in carriers attending daycare centres in Patras , Southwestern Greece .
	manualset3
221247	3	420639	7	NULL	NULL	0	NULL	serotype 6B Streptococcus pneumoniae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1996 , 19 isolates of serotype 6B Streptococcus pneumoniae with a unique resistance pattern were found in carriers attending daycare centres in Patras , Southwestern Greece .
	manualset3
221248	4	420639	7	NULL	NULL	0	NULL	unique resistance pattern	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1996 , 19 isolates of serotype 6B Streptococcus pneumoniae with a unique resistance pattern were found in carriers attending daycare centres in Patras , Southwestern Greece .
	manualset3
221249	5	420639	7	NULL	NULL	0	NULL	carriers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1996 , 19 isolates of serotype 6B Streptococcus pneumoniae with a unique resistance pattern were found in carriers attending daycare centres in Patras , Southwestern Greece .
	manualset3
221250	6	420639	7	NULL	NULL	0	NULL	daycare centres	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1996 , 19 isolates of serotype 6B Streptococcus pneumoniae with a unique resistance pattern were found in carriers attending daycare centres in Patras , Southwestern Greece .
	manualset3
221251	7	420639	7	NULL	NULL	0	NULL	Patras	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1996 , 19 isolates of serotype 6B Streptococcus pneumoniae with a unique resistance pattern were found in carriers attending daycare centres in Patras , Southwestern Greece .
	manualset3
221252	8	420639	7	NULL	NULL	0	NULL	Southwestern Greece 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1996 , 19 isolates of serotype 6B Streptococcus pneumoniae with a unique resistance pattern were found in carriers attending daycare centres in Patras , Southwestern Greece .
	manualset3
221253	1	420640	7	NULL	NULL	0	NULL	Cardiovascular responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Cardiovascular responses to microinjection of noradrenaline into the medial amygdaloid nucleus of conscious rats result from - receptor activation and vasopressin release .
	manualset3
221254	2	420640	7	NULL	NULL	0	NULL	microinjection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Cardiovascular responses to microinjection of noradrenaline into the medial amygdaloid nucleus of conscious rats result from - receptor activation and vasopressin release .
	manualset3
221255	3	420640	7	NULL	NULL	0	NULL	noradrenaline	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Cardiovascular responses to microinjection of noradrenaline into the medial amygdaloid nucleus of conscious rats result from - receptor activation and vasopressin release .
	manualset3
221256	4	420640	7	NULL	NULL	0	NULL	medial amygdaloid nucleus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Cardiovascular responses to microinjection of noradrenaline into the medial amygdaloid nucleus of conscious rats result from - receptor activation and vasopressin release .
	manualset3
221257	5	420640	7	NULL	NULL	0	NULL	conscious rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Cardiovascular responses to microinjection of noradrenaline into the medial amygdaloid nucleus of conscious rats result from - receptor activation and vasopressin release .
	manualset3
221258	6	420640	7	NULL	NULL	0	NULL	receptor activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cardiovascular responses to microinjection of noradrenaline into the medial amygdaloid nucleus of conscious rats result from - receptor activation and vasopressin release .
	manualset3
221259	7	420640	7	NULL	NULL	0	NULL	vasopressin release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cardiovascular responses to microinjection of noradrenaline into the medial amygdaloid nucleus of conscious rats result from - receptor activation and vasopressin release .
	manualset3
221260	1	420641	7	NULL	NULL	0	NULL	copper-ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The copper-ions released in VCu200 IUD users in different months were 2.61 , 1.98 , 1.96 , 1.82 , 1.22 , 1.20 , 1.15 , 0.98 ug/g .
	manualset3
221261	2	420641	7	NULL	NULL	0	NULL	VCu200 IUD users	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The copper-ions released in VCu200 IUD users in different months were 2.61 , 1.98 , 1.96 , 1.82 , 1.22 , 1.20 , 1.15 , 0.98 ug/g .
	manualset3
221262	3	420641	7	NULL	NULL	0	NULL	different months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The copper-ions released in VCu200 IUD users in different months were 2.61 , 1.98 , 1.96 , 1.82 , 1.22 , 1.20 , 1.15 , 0.98 ug/g .
	manualset3
221263	4	420641	7	NULL	NULL	0	NULL	2.61 ug/g	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The copper-ions released in VCu200 IUD users in different months were 2.61 , 1.98 , 1.96 , 1.82 , 1.22 , 1.20 , 1.15 , 0.98 ug/g .
	manualset3
221264	5	420641	7	NULL	NULL	0	NULL	1.98 ug/g	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The copper-ions released in VCu200 IUD users in different months were 2.61 , 1.98 , 1.96 , 1.82 , 1.22 , 1.20 , 1.15 , 0.98 ug/g .
	manualset3
221265	6	420641	7	NULL	NULL	0	NULL	1.96 ug/g	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The copper-ions released in VCu200 IUD users in different months were 2.61 , 1.98 , 1.96 , 1.82 , 1.22 , 1.20 , 1.15 , 0.98 ug/g .
	manualset3
221266	7	420641	7	NULL	NULL	0	NULL	1.82 ug/g	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The copper-ions released in VCu200 IUD users in different months were 2.61 , 1.98 , 1.96 , 1.82 , 1.22 , 1.20 , 1.15 , 0.98 ug/g .
	manualset3
221267	8	420641	7	NULL	NULL	0	NULL	1.22 ug/g	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The copper-ions released in VCu200 IUD users in different months were 2.61 , 1.98 , 1.96 , 1.82 , 1.22 , 1.20 , 1.15 , 0.98 ug/g .
	manualset3
221268	9	420641	7	NULL	NULL	0	NULL	1.20 ug/g	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The copper-ions released in VCu200 IUD users in different months were 2.61 , 1.98 , 1.96 , 1.82 , 1.22 , 1.20 , 1.15 , 0.98 ug/g .
	manualset3
221269	10	420641	7	NULL	NULL	0	NULL	1.15 ug/g	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The copper-ions released in VCu200 IUD users in different months were 2.61 , 1.98 , 1.96 , 1.82 , 1.22 , 1.20 , 1.15 , 0.98 ug/g .
	manualset3
221270	11	420641	7	NULL	NULL	0	NULL	0.98 ug/g	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The copper-ions released in VCu200 IUD users in different months were 2.61 , 1.98 , 1.96 , 1.82 , 1.22 , 1.20 , 1.15 , 0.98 ug/g .
	manualset3
221271	1	420642	7	NULL	NULL	0	NULL	questionnaire survey	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	We conducted a questionnaire survey among community and pharmaceutical company pharmacists in Lebanon to evaluate their satisfaction with their professional status and their willingness to work as clinical pharmacists .
	manualset3
221272	2	420642	7	NULL	NULL	0	NULL	community pharmacists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We conducted a questionnaire survey among community and pharmaceutical company pharmacists in Lebanon to evaluate their satisfaction with their professional status and their willingness to work as clinical pharmacists .
	manualset3
221273	3	420642	7	NULL	NULL	0	NULL	pharmaceutical company pharmacists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We conducted a questionnaire survey among community and pharmaceutical company pharmacists in Lebanon to evaluate their satisfaction with their professional status and their willingness to work as clinical pharmacists .
	manualset3
221274	4	420642	7	NULL	NULL	0	NULL	Lebanon	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	We conducted a questionnaire survey among community and pharmaceutical company pharmacists in Lebanon to evaluate their satisfaction with their professional status and their willingness to work as clinical pharmacists .
	manualset3
221275	5	420642	7	NULL	NULL	0	NULL	satisfaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We conducted a questionnaire survey among community and pharmaceutical company pharmacists in Lebanon to evaluate their satisfaction with their professional status and their willingness to work as clinical pharmacists .
	manualset3
221276	6	420642	7	NULL	NULL	0	NULL	professional status	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We conducted a questionnaire survey among community and pharmaceutical company pharmacists in Lebanon to evaluate their satisfaction with their professional status and their willingness to work as clinical pharmacists .
	manualset3
221277	7	420642	7	NULL	NULL	0	NULL	willingness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We conducted a questionnaire survey among community and pharmaceutical company pharmacists in Lebanon to evaluate their satisfaction with their professional status and their willingness to work as clinical pharmacists .
	manualset3
221278	8	420642	7	NULL	NULL	0	NULL	clinical pharmacists 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We conducted a questionnaire survey among community and pharmaceutical company pharmacists in Lebanon to evaluate their satisfaction with their professional status and their willingness to work as clinical pharmacists .
	manualset3
221279	1	420643	7	NULL	NULL	0	NULL	plateau phase cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In plateau phase cells a fluorescence band at 636 nm was predominant , which was further enhanced by increasing HpD concentration and/or increasing incubation time .
	manualset3
221280	2	420643	7	NULL	NULL	0	NULL	fluorescence band	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In plateau phase cells a fluorescence band at 636 nm was predominant , which was further enhanced by increasing HpD concentration and/or increasing incubation time .
	manualset3
221281	3	420643	7	NULL	NULL	0	NULL	 636 nm	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In plateau phase cells a fluorescence band at 636 nm was predominant , which was further enhanced by increasing HpD concentration and/or increasing incubation time .
	manualset3
221282	4	420643	7	NULL	NULL	0	NULL	HpD concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In plateau phase cells a fluorescence band at 636 nm was predominant , which was further enhanced by increasing HpD concentration and/or increasing incubation time .
	manualset3
221283	5	420643	7	NULL	NULL	0	NULL	incubation time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	In plateau phase cells a fluorescence band at 636 nm was predominant , which was further enhanced by increasing HpD concentration and/or increasing incubation time .
	manualset3
221284	1	420644	7	NULL	NULL	0	NULL	Dentinal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	( Dentinal cells and cavito-tubular system of teeth ) .
	manualset3
221285	2	420644	7	NULL	NULL	0	NULL	cavito-tubular system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Dentinal cells and cavito-tubular system of teeth ) .
	manualset3
221286	3	420644	7	NULL	NULL	0	NULL	teeth	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Dentinal cells and cavito-tubular system of teeth ) .
	manualset3
221287	1	420645	7	NULL	NULL	0	NULL	Ammonium leaching	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ammonium leaching was decreased by heat treatments in the most polluted soils , while CO2 was increased by heat in less polluted soils .
	manualset3
221288	2	420645	7	NULL	NULL	0	NULL	heat treatments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ammonium leaching was decreased by heat treatments in the most polluted soils , while CO2 was increased by heat in less polluted soils .
	manualset3
221289	3	420645	7	NULL	NULL	0	NULL	polluted soils	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Ammonium leaching was decreased by heat treatments in the most polluted soils , while CO2 was increased by heat in less polluted soils .
	manualset3
221290	4	420645	7	NULL	NULL	0	NULL	CO2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ammonium leaching was decreased by heat treatments in the most polluted soils , while CO2 was increased by heat in less polluted soils .
	manualset3
221291	5	420645	7	NULL	NULL	0	NULL	heat	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Ammonium leaching was decreased by heat treatments in the most polluted soils , while CO2 was increased by heat in less polluted soils .
	manualset3
221292	6	420645	7	NULL	NULL	0	NULL	less polluted soils 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Ammonium leaching was decreased by heat treatments in the most polluted soils , while CO2 was increased by heat in less polluted soils .
	manualset3
221293	1	420646	7	NULL	NULL	0	NULL	Pulmonary mechanics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary mechanics and plasma epinephrine and norepinephrine were measured before , at end exercise , and serially after each challenge .
	manualset3
221294	2	420646	7	NULL	NULL	0	NULL	plasma epinephrine 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary mechanics and plasma epinephrine and norepinephrine were measured before , at end exercise , and serially after each challenge .
	manualset3
221295	3	420646	7	NULL	NULL	0	NULL	norepinephrine	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary mechanics and plasma epinephrine and norepinephrine were measured before , at end exercise , and serially after each challenge .
	manualset3
221296	4	420646	7	NULL	NULL	0	NULL	exercise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary mechanics and plasma epinephrine and norepinephrine were measured before , at end exercise , and serially after each challenge .
	manualset3
221297	5	420646	7	NULL	NULL	0	NULL	challenge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pulmonary mechanics and plasma epinephrine and norepinephrine were measured before , at end exercise , and serially after each challenge .
	manualset3
221298	1	420647	7	NULL	NULL	0	NULL	Coculture	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Coculture of fluorescently labeled VHL-deficient and VHL-positive cells showed discriminate killing of the VHL-deficient cells with ChA3 .
	manualset3
221299	2	420647	7	NULL	NULL	0	NULL	fluorescently labeled VHL-deficient cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Coculture of fluorescently labeled VHL-deficient and VHL-positive cells showed discriminate killing of the VHL-deficient cells with ChA3 .
	manualset3
221300	3	420647	7	NULL	NULL	0	NULL	VHL-positive cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Coculture of fluorescently labeled VHL-deficient and VHL-positive cells showed discriminate killing of the VHL-deficient cells with ChA3 .
	manualset3
221301	4	420647	7	NULL	NULL	0	NULL	 killing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Coculture of fluorescently labeled VHL-deficient and VHL-positive cells showed discriminate killing of the VHL-deficient cells with ChA3 .
	manualset3
221302	5	420647	7	NULL	NULL	0	NULL	VHL-deficient cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Coculture of fluorescently labeled VHL-deficient and VHL-positive cells showed discriminate killing of the VHL-deficient cells with ChA3 .
	manualset3
221303	6	420647	7	NULL	NULL	0	NULL	ChA3	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Coculture of fluorescently labeled VHL-deficient and VHL-positive cells showed discriminate killing of the VHL-deficient cells with ChA3 .
	manualset3
221313	1	420648	7	NULL	NULL	0	NULL	Free flaps	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Free flaps may safely allow meaningful ambulation , durable limb preservation , and better quality of life in patients undergoing resections of soft-tissue cancers of the foot .
	manualset3
221315	2	420648	7	NULL	NULL	0	NULL	meaningful ambulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Free flaps may safely allow meaningful ambulation , durable limb preservation , and better quality of life in patients undergoing resections of soft-tissue cancers of the foot .
	manualset3
221317	3	420648	7	NULL	NULL	0	NULL	durable limb preservation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Free flaps may safely allow meaningful ambulation , durable limb preservation , and better quality of life in patients undergoing resections of soft-tissue cancers of the foot .
	manualset3
221318	4	420648	7	NULL	NULL	0	NULL	quality of life	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Free flaps may safely allow meaningful ambulation , durable limb preservation , and better quality of life in patients undergoing resections of soft-tissue cancers of the foot .
	manualset3
221320	5	420648	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Free flaps may safely allow meaningful ambulation , durable limb preservation , and better quality of life in patients undergoing resections of soft-tissue cancers of the foot .
	manualset3
221321	6	420648	7	NULL	NULL	0	NULL	resections	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Free flaps may safely allow meaningful ambulation , durable limb preservation , and better quality of life in patients undergoing resections of soft-tissue cancers of the foot .
	manualset3
221323	7	420648	7	NULL	NULL	0	NULL	soft-tissue cancers	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Free flaps may safely allow meaningful ambulation , durable limb preservation , and better quality of life in patients undergoing resections of soft-tissue cancers of the foot .
	manualset3
221324	8	420648	7	NULL	NULL	0	NULL	foot 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Free flaps may safely allow meaningful ambulation , durable limb preservation , and better quality of life in patients undergoing resections of soft-tissue cancers of the foot .
	manualset3
221326	1	420649	7	NULL	NULL	0	NULL	Surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Surgery via natural orifices in human beings : yesterday , today , tomorrow .
	manualset3
221328	2	420649	7	NULL	NULL	0	NULL	natural orifices	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Surgery via natural orifices in human beings : yesterday , today , tomorrow .
	manualset3
221329	3	420649	7	NULL	NULL	0	NULL	human beings	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Surgery via natural orifices in human beings : yesterday , today , tomorrow .
	manualset3
221331	4	420649	7	NULL	NULL	0	NULL	yesterday	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Surgery via natural orifices in human beings : yesterday , today , tomorrow .
	manualset3
221332	5	420649	7	NULL	NULL	0	NULL	today	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Surgery via natural orifices in human beings : yesterday , today , tomorrow .
	manualset3
221334	6	420649	7	NULL	NULL	0	NULL	 tomorrow	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Surgery via natural orifices in human beings : yesterday , today , tomorrow .
	manualset3
221337	1	420650	7	NULL	NULL	0	NULL	high-performance liquid chromatographic ( HPLC ) method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A high-performance liquid chromatographic ( HPLC ) method for the determination of the ionophore coccidiostat lasalocid in poultry muscle and eggs was developed .
	manualset3
221338	2	420650	7	NULL	NULL	0	NULL	determination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A high-performance liquid chromatographic ( HPLC ) method for the determination of the ionophore coccidiostat lasalocid in poultry muscle and eggs was developed .
	manualset3
221340	3	420650	7	NULL	NULL	0	NULL	 ionophore	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A high-performance liquid chromatographic ( HPLC ) method for the determination of the ionophore coccidiostat lasalocid in poultry muscle and eggs was developed .
	manualset3
221341	4	420650	7	NULL	NULL	0	NULL	coccidiostat lasalocid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A high-performance liquid chromatographic ( HPLC ) method for the determination of the ionophore coccidiostat lasalocid in poultry muscle and eggs was developed .
	manualset3
221342	5	420650	7	NULL	NULL	0	NULL	poultry muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A high-performance liquid chromatographic ( HPLC ) method for the determination of the ionophore coccidiostat lasalocid in poultry muscle and eggs was developed .
	manualset3
221343	6	420650	7	NULL	NULL	0	NULL	eggs 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A high-performance liquid chromatographic ( HPLC ) method for the determination of the ionophore coccidiostat lasalocid in poultry muscle and eggs was developed .
	manualset3
221344	1	420651	7	NULL	NULL	0	NULL	impressive developments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the impressive developments in the last decades , several protocols for catalytic oxidation are today available , which are based on the extraordinary properties of gold in terms of catalytic activity , selectivity , reusability and resistance to poisons .
	manualset3
221345	2	420651	7	NULL	NULL	0	NULL	last decades	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the impressive developments in the last decades , several protocols for catalytic oxidation are today available , which are based on the extraordinary properties of gold in terms of catalytic activity , selectivity , reusability and resistance to poisons .
	manualset3
221346	3	420651	7	NULL	NULL	0	NULL	protocols	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the impressive developments in the last decades , several protocols for catalytic oxidation are today available , which are based on the extraordinary properties of gold in terms of catalytic activity , selectivity , reusability and resistance to poisons .
	manualset3
221347	4	420651	7	NULL	NULL	0	NULL	catalytic oxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the impressive developments in the last decades , several protocols for catalytic oxidation are today available , which are based on the extraordinary properties of gold in terms of catalytic activity , selectivity , reusability and resistance to poisons .
	manualset3
221348	5	420651	7	NULL	NULL	0	NULL	extraordinary properties	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the impressive developments in the last decades , several protocols for catalytic oxidation are today available , which are based on the extraordinary properties of gold in terms of catalytic activity , selectivity , reusability and resistance to poisons .
	manualset3
221349	6	420651	7	NULL	NULL	0	NULL	gold	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the impressive developments in the last decades , several protocols for catalytic oxidation are today available , which are based on the extraordinary properties of gold in terms of catalytic activity , selectivity , reusability and resistance to poisons .
	manualset3
221350	7	420651	7	NULL	NULL	0	NULL	catalytic activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the impressive developments in the last decades , several protocols for catalytic oxidation are today available , which are based on the extraordinary properties of gold in terms of catalytic activity , selectivity , reusability and resistance to poisons .
	manualset3
221351	8	420651	7	NULL	NULL	0	NULL	selectivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the impressive developments in the last decades , several protocols for catalytic oxidation are today available , which are based on the extraordinary properties of gold in terms of catalytic activity , selectivity , reusability and resistance to poisons .
	manualset3
221352	9	420651	7	NULL	NULL	0	NULL	reusability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the impressive developments in the last decades , several protocols for catalytic oxidation are today available , which are based on the extraordinary properties of gold in terms of catalytic activity , selectivity , reusability and resistance to poisons .
	manualset3
221353	10	420651	7	NULL	NULL	0	NULL	resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the impressive developments in the last decades , several protocols for catalytic oxidation are today available , which are based on the extraordinary properties of gold in terms of catalytic activity , selectivity , reusability and resistance to poisons .
	manualset3
221354	11	420651	7	NULL	NULL	0	NULL	poisons	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the impressive developments in the last decades , several protocols for catalytic oxidation are today available , which are based on the extraordinary properties of gold in terms of catalytic activity , selectivity , reusability and resistance to poisons .
	manualset3
221356	1	420652	7	NULL	NULL	0	NULL	 unilateral process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The unilateral process of informed consent is evolving into one of informed collaborative choice .
	manualset3
221357	2	420652	7	NULL	NULL	0	NULL	informed consent	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The unilateral process of informed consent is evolving into one of informed collaborative choice .
	manualset3
221358	3	420652	7	NULL	NULL	0	NULL	 one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The unilateral process of informed consent is evolving into one of informed collaborative choice .
	manualset3
221360	4	420652	7	NULL	NULL	0	NULL	collaborative choice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The unilateral process of informed consent is evolving into one of informed collaborative choice .
	manualset3
221362	1	420653	7	NULL	NULL	0	NULL	11 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 11 G. vaginalis strains tested , all showed antagonistic activity against at least one of the 22 indicator bacteria assayed .
	manualset3
221365	2	420653	7	NULL	NULL	0	NULL	G. vaginalis strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 11 G. vaginalis strains tested , all showed antagonistic activity against at least one of the 22 indicator bacteria assayed .
	manualset3
221366	3	420653	7	NULL	NULL	0	NULL	antagonistic activity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 11 G. vaginalis strains tested , all showed antagonistic activity against at least one of the 22 indicator bacteria assayed .
	manualset3
221368	4	420653	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 11 G. vaginalis strains tested , all showed antagonistic activity against at least one of the 22 indicator bacteria assayed .
	manualset3
221369	5	420653	7	NULL	NULL	0	NULL	22 indicator bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 11 G. vaginalis strains tested , all showed antagonistic activity against at least one of the 22 indicator bacteria assayed .
	manualset3
221372	1	420654	7	NULL	NULL	0	NULL	MDA modification	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MDA modification of Arg oligomers not only resulted in improved detection sensitivity for most of the peptides studied ( e. g. , more than six-fold for Arg ( 7 ) ) , but also greatly enhanced the quality of MS/MS spectra , in line with previous results for other peptides .
	manualset3
221374	2	420654	7	NULL	NULL	0	NULL	Arg oligomers	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	MDA modification of Arg oligomers not only resulted in improved detection sensitivity for most of the peptides studied ( e. g. , more than six-fold for Arg ( 7 ) ) , but also greatly enhanced the quality of MS/MS spectra , in line with previous results for other peptides .
	manualset3
221376	3	420654	7	NULL	NULL	0	NULL	improved detection sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MDA modification of Arg oligomers not only resulted in improved detection sensitivity for most of the peptides studied ( e. g. , more than six-fold for Arg ( 7 ) ) , but also greatly enhanced the quality of MS/MS spectra , in line with previous results for other peptides .
	manualset3
221378	4	420654	7	NULL	NULL	0	NULL	 peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	MDA modification of Arg oligomers not only resulted in improved detection sensitivity for most of the peptides studied ( e. g. , more than six-fold for Arg ( 7 ) ) , but also greatly enhanced the quality of MS/MS spectra , in line with previous results for other peptides .
	manualset3
221380	5	420654	7	NULL	NULL	0	NULL	six-fold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	MDA modification of Arg oligomers not only resulted in improved detection sensitivity for most of the peptides studied ( e. g. , more than six-fold for Arg ( 7 ) ) , but also greatly enhanced the quality of MS/MS spectra , in line with previous results for other peptides .
	manualset3
221381	6	420654	7	NULL	NULL	0	NULL	Arg ( 7 ) 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	MDA modification of Arg oligomers not only resulted in improved detection sensitivity for most of the peptides studied ( e. g. , more than six-fold for Arg ( 7 ) ) , but also greatly enhanced the quality of MS/MS spectra , in line with previous results for other peptides .
	manualset3
221383	7	420654	7	NULL	NULL	0	NULL	quality 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	MDA modification of Arg oligomers not only resulted in improved detection sensitivity for most of the peptides studied ( e. g. , more than six-fold for Arg ( 7 ) ) , but also greatly enhanced the quality of MS/MS spectra , in line with previous results for other peptides .
	manualset3
221385	8	420654	7	NULL	NULL	0	NULL	MS/MS spectra	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	MDA modification of Arg oligomers not only resulted in improved detection sensitivity for most of the peptides studied ( e. g. , more than six-fold for Arg ( 7 ) ) , but also greatly enhanced the quality of MS/MS spectra , in line with previous results for other peptides .
	manualset3
221386	9	420654	7	NULL	NULL	0	NULL	previous results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MDA modification of Arg oligomers not only resulted in improved detection sensitivity for most of the peptides studied ( e. g. , more than six-fold for Arg ( 7 ) ) , but also greatly enhanced the quality of MS/MS spectra , in line with previous results for other peptides .
	manualset3
221388	10	420654	7	NULL	NULL	0	NULL	peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	MDA modification of Arg oligomers not only resulted in improved detection sensitivity for most of the peptides studied ( e. g. , more than six-fold for Arg ( 7 ) ) , but also greatly enhanced the quality of MS/MS spectra , in line with previous results for other peptides .
	manualset3
221391	1	420655	7	NULL	NULL	0	NULL	Outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcome in adult ALL is still unsatisfactory , which is due to less cumulative dosing of chemotherapy and less strict adherence to timing of successive cycles .
	manualset3
221392	2	420655	7	NULL	NULL	0	NULL	adult ALL	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcome in adult ALL is still unsatisfactory , which is due to less cumulative dosing of chemotherapy and less strict adherence to timing of successive cycles .
	manualset3
221393	3	420655	7	NULL	NULL	0	NULL	cumulative dosing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcome in adult ALL is still unsatisfactory , which is due to less cumulative dosing of chemotherapy and less strict adherence to timing of successive cycles .
	manualset3
221394	4	420655	7	NULL	NULL	0	NULL	chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcome in adult ALL is still unsatisfactory , which is due to less cumulative dosing of chemotherapy and less strict adherence to timing of successive cycles .
	manualset3
221395	5	420655	7	NULL	NULL	0	NULL	less strict adherence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcome in adult ALL is still unsatisfactory , which is due to less cumulative dosing of chemotherapy and less strict adherence to timing of successive cycles .
	manualset3
221396	6	420655	7	NULL	NULL	0	NULL	timing 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcome in adult ALL is still unsatisfactory , which is due to less cumulative dosing of chemotherapy and less strict adherence to timing of successive cycles .
	manualset3
221397	7	420655	7	NULL	NULL	0	NULL	successive cycles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Outcome in adult ALL is still unsatisfactory , which is due to less cumulative dosing of chemotherapy and less strict adherence to timing of successive cycles .
	manualset3
221398	1	420656	7	NULL	NULL	0	NULL	Supramolecular double helix 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Supramolecular double helix from capped - peptide .
	manualset3
221399	2	420656	7	NULL	NULL	0	NULL	capped - peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Supramolecular double helix from capped - peptide .
	manualset3
221400	1	420657	7	NULL	NULL	0	NULL	Asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Asthma with sulfite intolerance in children : a blocking study with cyanocobalamin .
	manualset3
221401	2	420657	7	NULL	NULL	0	NULL	sulfite intolerance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Asthma with sulfite intolerance in children : a blocking study with cyanocobalamin .
	manualset3
221402	3	420657	7	NULL	NULL	0	NULL	 children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Asthma with sulfite intolerance in children : a blocking study with cyanocobalamin .
	manualset3
221403	4	420657	7	NULL	NULL	0	NULL	blocking study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Asthma with sulfite intolerance in children : a blocking study with cyanocobalamin .
	manualset3
221404	5	420657	7	NULL	NULL	NULL	NULL	cyanocobalamin	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Asthma with sulfite intolerance in children : a blocking study with cyanocobalamin .
	manualset3
221405	1	420658	7	NULL	NULL	0	NULL	Effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Effect of leukocyte hydrolases on bacteria .
	manualset3
221406	2	420658	7	NULL	NULL	0	NULL	leukocyte hydrolases 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Effect of leukocyte hydrolases on bacteria .
	manualset3
221407	3	420658	7	NULL	NULL	0	NULL	 bacteria 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Effect of leukocyte hydrolases on bacteria .
	manualset3
221410	1	420659	7	NULL	NULL	0	NULL	Ultracentrifugal boundaries	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultracentrifugal boundaries corresponding to those seen in the original extracts were present , the main component having an s20 , ( w ) of 81 S. Upon exposure to chelating agents , the particles dissociated through an intermediate component with sedimentation rate of 56 S to a final stage in which 46 and 28 S subunits were present in a weight ratio of 2 : 1 .
	manualset3
221413	2	420659	7	NULL	NULL	0	NULL	original extracts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultracentrifugal boundaries corresponding to those seen in the original extracts were present , the main component having an s20 , ( w ) of 81 S. Upon exposure to chelating agents , the particles dissociated through an intermediate component with sedimentation rate of 56 S to a final stage in which 46 and 28 S subunits were present in a weight ratio of 2 : 1 .
	manualset3
221415	3	420659	7	NULL	NULL	0	NULL	main component	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultracentrifugal boundaries corresponding to those seen in the original extracts were present , the main component having an s20 , ( w ) of 81 S. Upon exposure to chelating agents , the particles dissociated through an intermediate component with sedimentation rate of 56 S to a final stage in which 46 and 28 S subunits were present in a weight ratio of 2 : 1 .
	manualset3
221416	4	420659	7	NULL	NULL	0	NULL	 s20	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultracentrifugal boundaries corresponding to those seen in the original extracts were present , the main component having an s20 , ( w ) of 81 S. Upon exposure to chelating agents , the particles dissociated through an intermediate component with sedimentation rate of 56 S to a final stage in which 46 and 28 S subunits were present in a weight ratio of 2 : 1 .
	manualset3
221417	5	420659	7	NULL	NULL	0	NULL	( w ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultracentrifugal boundaries corresponding to those seen in the original extracts were present , the main component having an s20 , ( w ) of 81 S. Upon exposure to chelating agents , the particles dissociated through an intermediate component with sedimentation rate of 56 S to a final stage in which 46 and 28 S subunits were present in a weight ratio of 2 : 1 .
	manualset3
221419	6	420659	7	NULL	NULL	0	NULL	81 S	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultracentrifugal boundaries corresponding to those seen in the original extracts were present , the main component having an s20 , ( w ) of 81 S. Upon exposure to chelating agents , the particles dissociated through an intermediate component with sedimentation rate of 56 S to a final stage in which 46 and 28 S subunits were present in a weight ratio of 2 : 1 .
	manualset3
221420	7	420659	7	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultracentrifugal boundaries corresponding to those seen in the original extracts were present , the main component having an s20 , ( w ) of 81 S. Upon exposure to chelating agents , the particles dissociated through an intermediate component with sedimentation rate of 56 S to a final stage in which 46 and 28 S subunits were present in a weight ratio of 2 : 1 .
	manualset3
221422	8	420659	7	NULL	NULL	0	NULL	chelating agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultracentrifugal boundaries corresponding to those seen in the original extracts were present , the main component having an s20 , ( w ) of 81 S. Upon exposure to chelating agents , the particles dissociated through an intermediate component with sedimentation rate of 56 S to a final stage in which 46 and 28 S subunits were present in a weight ratio of 2 : 1 .
	manualset3
221423	9	420659	7	NULL	NULL	0	NULL	particles	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultracentrifugal boundaries corresponding to those seen in the original extracts were present , the main component having an s20 , ( w ) of 81 S. Upon exposure to chelating agents , the particles dissociated through an intermediate component with sedimentation rate of 56 S to a final stage in which 46 and 28 S subunits were present in a weight ratio of 2 : 1 .
	manualset3
221424	10	420659	7	NULL	NULL	0	NULL	intermediate component	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultracentrifugal boundaries corresponding to those seen in the original extracts were present , the main component having an s20 , ( w ) of 81 S. Upon exposure to chelating agents , the particles dissociated through an intermediate component with sedimentation rate of 56 S to a final stage in which 46 and 28 S subunits were present in a weight ratio of 2 : 1 .
	manualset3
221425	11	420659	7	NULL	NULL	0	NULL	sedimentation rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultracentrifugal boundaries corresponding to those seen in the original extracts were present , the main component having an s20 , ( w ) of 81 S. Upon exposure to chelating agents , the particles dissociated through an intermediate component with sedimentation rate of 56 S to a final stage in which 46 and 28 S subunits were present in a weight ratio of 2 : 1 .
	manualset3
221426	12	420659	7	NULL	NULL	0	NULL	56 S	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultracentrifugal boundaries corresponding to those seen in the original extracts were present , the main component having an s20 , ( w ) of 81 S. Upon exposure to chelating agents , the particles dissociated through an intermediate component with sedimentation rate of 56 S to a final stage in which 46 and 28 S subunits were present in a weight ratio of 2 : 1 .
	manualset3
221427	13	420659	7	NULL	NULL	0	NULL	final stage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultracentrifugal boundaries corresponding to those seen in the original extracts were present , the main component having an s20 , ( w ) of 81 S. Upon exposure to chelating agents , the particles dissociated through an intermediate component with sedimentation rate of 56 S to a final stage in which 46 and 28 S subunits were present in a weight ratio of 2 : 1 .
	manualset3
221428	14	420659	7	NULL	NULL	0	NULL	 46S subunits	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultracentrifugal boundaries corresponding to those seen in the original extracts were present , the main component having an s20 , ( w ) of 81 S. Upon exposure to chelating agents , the particles dissociated through an intermediate component with sedimentation rate of 56 S to a final stage in which 46 and 28 S subunits were present in a weight ratio of 2 : 1 .
	manualset3
221429	15	420659	7	NULL	NULL	0	NULL	28 S subunits	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultracentrifugal boundaries corresponding to those seen in the original extracts were present , the main component having an s20 , ( w ) of 81 S. Upon exposure to chelating agents , the particles dissociated through an intermediate component with sedimentation rate of 56 S to a final stage in which 46 and 28 S subunits were present in a weight ratio of 2 : 1 .
	manualset3
221430	16	420659	7	NULL	NULL	0	NULL	weight ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultracentrifugal boundaries corresponding to those seen in the original extracts were present , the main component having an s20 , ( w ) of 81 S. Upon exposure to chelating agents , the particles dissociated through an intermediate component with sedimentation rate of 56 S to a final stage in which 46 and 28 S subunits were present in a weight ratio of 2 : 1 .
	manualset3
221431	17	420659	7	NULL	NULL	0	NULL	2 : 1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultracentrifugal boundaries corresponding to those seen in the original extracts were present , the main component having an s20 , ( w ) of 81 S. Upon exposure to chelating agents , the particles dissociated through an intermediate component with sedimentation rate of 56 S to a final stage in which 46 and 28 S subunits were present in a weight ratio of 2 : 1 .
	manualset3
221432	1	420660	7	NULL	NULL	0	NULL	Implications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Implications for sport participation promotion are discussed .
	manualset3
221433	2	420660	7	NULL	NULL	0	NULL	sport participation promotion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Implications for sport participation promotion are discussed .
	manualset3
221434	1	420661	7	NULL	NULL	0	NULL	132 such specimens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 132 such specimens , NV was detected in only one .
	manualset3
221435	2	420661	7	NULL	NULL	0	NULL	NV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 132 such specimens , NV was detected in only one .
	manualset3
221436	3	420661	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 132 such specimens , NV was detected in only one .
	manualset3
221437	1	420662	7	NULL	NULL	0	NULL	Protoplasmic streaming	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Protoplasmic streaming as a process of jet propulsion .
	manualset3
221438	2	420662	7	NULL	NULL	0	NULL	 process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Protoplasmic streaming as a process of jet propulsion .
	manualset3
221439	3	420662	7	NULL	NULL	0	NULL	jet propulsion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Protoplasmic streaming as a process of jet propulsion .
	manualset3
221440	1	420663	7	NULL	NULL	0	NULL	 Disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Disorders following the consumption of food from communal kitchens , based on a 10-year analysis ) .
	manualset3
221441	2	420663	7	NULL	NULL	0	NULL	consumption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Disorders following the consumption of food from communal kitchens , based on a 10-year analysis ) .
	manualset3
221442	3	420663	7	NULL	NULL	0	NULL	 food	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	( Disorders following the consumption of food from communal kitchens , based on a 10-year analysis ) .
	manualset3
221443	4	420663	7	NULL	NULL	0	NULL	communal kitchens	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( Disorders following the consumption of food from communal kitchens , based on a 10-year analysis ) .
	manualset3
221444	5	420663	7	NULL	NULL	0	NULL	10-year analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Disorders following the consumption of food from communal kitchens , based on a 10-year analysis ) .
	manualset3
221445	1	420664	7	NULL	NULL	0	NULL	Operative dentistry	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Operative dentistry and endodontics of the physically limited patient .
	manualset3
221446	2	420664	7	NULL	NULL	0	NULL	endodontics	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Operative dentistry and endodontics of the physically limited patient .
	manualset3
221447	3	420664	7	NULL	NULL	0	NULL	physically limited patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Operative dentistry and endodontics of the physically limited patient .
	manualset3
221448	1	420665	7	NULL	NULL	0	NULL	Digestibilities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Digestibilities of fatty acids and other nutrient fractions and characteristics of ruminal fluid generally were similar between flaked and prilled fatty acids , despite the larger particle size of flaked fatty acids .
	manualset3
221449	2	420665	7	NULL	NULL	0	NULL	fatty acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Digestibilities of fatty acids and other nutrient fractions and characteristics of ruminal fluid generally were similar between flaked and prilled fatty acids , despite the larger particle size of flaked fatty acids .
	manualset3
221450	3	420665	7	NULL	NULL	0	NULL	nutrient fractions	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Digestibilities of fatty acids and other nutrient fractions and characteristics of ruminal fluid generally were similar between flaked and prilled fatty acids , despite the larger particle size of flaked fatty acids .
	manualset3
221451	4	420665	7	NULL	NULL	0	NULL	characteristics	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Digestibilities of fatty acids and other nutrient fractions and characteristics of ruminal fluid generally were similar between flaked and prilled fatty acids , despite the larger particle size of flaked fatty acids .
	manualset3
221452	5	420665	7	NULL	NULL	0	NULL	ruminal fluid	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Digestibilities of fatty acids and other nutrient fractions and characteristics of ruminal fluid generally were similar between flaked and prilled fatty acids , despite the larger particle size of flaked fatty acids .
	manualset3
221453	6	420665	7	NULL	NULL	0	NULL	flaked fatty acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Digestibilities of fatty acids and other nutrient fractions and characteristics of ruminal fluid generally were similar between flaked and prilled fatty acids , despite the larger particle size of flaked fatty acids .
	manualset3
221454	7	420665	7	NULL	NULL	0	NULL	prilled fatty acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Digestibilities of fatty acids and other nutrient fractions and characteristics of ruminal fluid generally were similar between flaked and prilled fatty acids , despite the larger particle size of flaked fatty acids .
	manualset3
221455	8	420665	7	NULL	NULL	0	NULL	larger particle size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Digestibilities of fatty acids and other nutrient fractions and characteristics of ruminal fluid generally were similar between flaked and prilled fatty acids , despite the larger particle size of flaked fatty acids .
	manualset3
221456	9	420665	7	NULL	NULL	0	NULL	flaked fatty acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Digestibilities of fatty acids and other nutrient fractions and characteristics of ruminal fluid generally were similar between flaked and prilled fatty acids , despite the larger particle size of flaked fatty acids .
	manualset3
221457	1	420666	7	NULL	NULL	0	NULL	Pro conservative long-term therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Pro conservative long-term therapy of peptic ulcer ) .
	manualset3
221458	2	420666	7	NULL	NULL	0	NULL	peptic ulcer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Pro conservative long-term therapy of peptic ulcer ) .
	manualset3
221459	1	420667	7	NULL	NULL	0	NULL	Comparison	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of extracellular protein profiles of P. syringae pv .
	manualset3
221460	2	420667	7	NULL	NULL	0	NULL	extracellular protein profiles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of extracellular protein profiles of P. syringae pv .
	manualset3
221461	3	420667	7	NULL	NULL	0	NULL	P. syringae pv 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of extracellular protein profiles of P. syringae pv .
	manualset3
221462	1	420668	7	NULL	NULL	0	NULL	parallel changes 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We infer that parallel changes in melanization and desiccation resistance may result from decreasing annual average temperature and relative humidity along increasing latitude as well as altitude on the Indian subcontinent .
	manualset3
221463	2	420668	7	NULL	NULL	0	NULL	melanization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We infer that parallel changes in melanization and desiccation resistance may result from decreasing annual average temperature and relative humidity along increasing latitude as well as altitude on the Indian subcontinent .
	manualset3
221464	3	420668	7	NULL	NULL	0	NULL	desiccation resistance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We infer that parallel changes in melanization and desiccation resistance may result from decreasing annual average temperature and relative humidity along increasing latitude as well as altitude on the Indian subcontinent .
	manualset3
221465	4	420668	7	NULL	NULL	0	NULL	decreasing annual average temperature	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We infer that parallel changes in melanization and desiccation resistance may result from decreasing annual average temperature and relative humidity along increasing latitude as well as altitude on the Indian subcontinent .
	manualset3
221466	5	420668	7	NULL	NULL	0	NULL	relative humidity	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We infer that parallel changes in melanization and desiccation resistance may result from decreasing annual average temperature and relative humidity along increasing latitude as well as altitude on the Indian subcontinent .
	manualset3
221467	6	420668	7	NULL	NULL	0	NULL	increasing latitude 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We infer that parallel changes in melanization and desiccation resistance may result from decreasing annual average temperature and relative humidity along increasing latitude as well as altitude on the Indian subcontinent .
	manualset3
221468	7	420668	7	NULL	NULL	0	NULL	altitude	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We infer that parallel changes in melanization and desiccation resistance may result from decreasing annual average temperature and relative humidity along increasing latitude as well as altitude on the Indian subcontinent .
	manualset3
221469	8	420668	7	NULL	NULL	0	NULL	Indian subcontinent	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	We infer that parallel changes in melanization and desiccation resistance may result from decreasing annual average temperature and relative humidity along increasing latitude as well as altitude on the Indian subcontinent .
	manualset3
221470	1	420669	7	NULL	NULL	0	NULL	Media multitasking	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Media multitasking was also associated with negative social indicators .
	manualset3
221471	2	420669	7	NULL	NULL	NULL	NULL	negative social indicators 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Media multitasking was also associated with negative social indicators .
	manualset3
221472	1	420670	7	NULL	NULL	0	NULL	Chronic fatigue immune dysfunction syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic fatigue immune dysfunction syndrome : an epidemic ?
	manualset3
221473	2	420670	7	NULL	NULL	0	NULL	epidemic 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic fatigue immune dysfunction syndrome : an epidemic ?
	manualset3
221474	1	420671	7	NULL	NULL	0	NULL	14 focus reduction neutralization test-positive sera	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 14 focus reduction neutralization test-positive sera , specific reactivity ( at least 4-fold higher endpoint titer ) of neutralizing antibodies was as follows : six sera were specific for Saaremaa hantavirus , three showed equal titers to Saaremaa and Dobrava hantaviruses , and five showed the highest endpoint titers to Puumala hantavirus .
	manualset3
221475	2	420671	7	NULL	NULL	0	NULL	specific reactivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 14 focus reduction neutralization test-positive sera , specific reactivity ( at least 4-fold higher endpoint titer ) of neutralizing antibodies was as follows : six sera were specific for Saaremaa hantavirus , three showed equal titers to Saaremaa and Dobrava hantaviruses , and five showed the highest endpoint titers to Puumala hantavirus .
	manualset3
221476	3	420671	7	NULL	NULL	0	NULL	4-fold higher endpoint titer	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 14 focus reduction neutralization test-positive sera , specific reactivity ( at least 4-fold higher endpoint titer ) of neutralizing antibodies was as follows : six sera were specific for Saaremaa hantavirus , three showed equal titers to Saaremaa and Dobrava hantaviruses , and five showed the highest endpoint titers to Puumala hantavirus .
	manualset3
221477	4	420671	7	NULL	NULL	0	NULL	neutralizing antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 14 focus reduction neutralization test-positive sera , specific reactivity ( at least 4-fold higher endpoint titer ) of neutralizing antibodies was as follows : six sera were specific for Saaremaa hantavirus , three showed equal titers to Saaremaa and Dobrava hantaviruses , and five showed the highest endpoint titers to Puumala hantavirus .
	manualset3
221478	5	420671	7	NULL	NULL	0	NULL	six sera	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 14 focus reduction neutralization test-positive sera , specific reactivity ( at least 4-fold higher endpoint titer ) of neutralizing antibodies was as follows : six sera were specific for Saaremaa hantavirus , three showed equal titers to Saaremaa and Dobrava hantaviruses , and five showed the highest endpoint titers to Puumala hantavirus .
	manualset3
221479	6	420671	7	NULL	NULL	0	NULL	Saaremaa hantavirus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 14 focus reduction neutralization test-positive sera , specific reactivity ( at least 4-fold higher endpoint titer ) of neutralizing antibodies was as follows : six sera were specific for Saaremaa hantavirus , three showed equal titers to Saaremaa and Dobrava hantaviruses , and five showed the highest endpoint titers to Puumala hantavirus .
	manualset3
221480	7	420671	7	NULL	NULL	0	NULL	three 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 14 focus reduction neutralization test-positive sera , specific reactivity ( at least 4-fold higher endpoint titer ) of neutralizing antibodies was as follows : six sera were specific for Saaremaa hantavirus , three showed equal titers to Saaremaa and Dobrava hantaviruses , and five showed the highest endpoint titers to Puumala hantavirus .
	manualset3
221481	8	420671	7	NULL	NULL	0	NULL	 equal titers	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 14 focus reduction neutralization test-positive sera , specific reactivity ( at least 4-fold higher endpoint titer ) of neutralizing antibodies was as follows : six sera were specific for Saaremaa hantavirus , three showed equal titers to Saaremaa and Dobrava hantaviruses , and five showed the highest endpoint titers to Puumala hantavirus .
	manualset3
221482	9	420671	7	NULL	NULL	0	NULL	Saaremaa hantavirus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 14 focus reduction neutralization test-positive sera , specific reactivity ( at least 4-fold higher endpoint titer ) of neutralizing antibodies was as follows : six sera were specific for Saaremaa hantavirus , three showed equal titers to Saaremaa and Dobrava hantaviruses , and five showed the highest endpoint titers to Puumala hantavirus .
	manualset3
221483	10	420671	7	NULL	NULL	0	NULL	Dobrava hantaviruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 14 focus reduction neutralization test-positive sera , specific reactivity ( at least 4-fold higher endpoint titer ) of neutralizing antibodies was as follows : six sera were specific for Saaremaa hantavirus , three showed equal titers to Saaremaa and Dobrava hantaviruses , and five showed the highest endpoint titers to Puumala hantavirus .
	manualset3
221484	11	420671	7	NULL	NULL	0	NULL	five	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 14 focus reduction neutralization test-positive sera , specific reactivity ( at least 4-fold higher endpoint titer ) of neutralizing antibodies was as follows : six sera were specific for Saaremaa hantavirus , three showed equal titers to Saaremaa and Dobrava hantaviruses , and five showed the highest endpoint titers to Puumala hantavirus .
	manualset3
221485	12	420671	7	NULL	NULL	0	NULL	endpoint titers 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 14 focus reduction neutralization test-positive sera , specific reactivity ( at least 4-fold higher endpoint titer ) of neutralizing antibodies was as follows : six sera were specific for Saaremaa hantavirus , three showed equal titers to Saaremaa and Dobrava hantaviruses , and five showed the highest endpoint titers to Puumala hantavirus .
	manualset3
221486	13	420671	7	NULL	NULL	0	NULL	Puumala hantavirus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 14 focus reduction neutralization test-positive sera , specific reactivity ( at least 4-fold higher endpoint titer ) of neutralizing antibodies was as follows : six sera were specific for Saaremaa hantavirus , three showed equal titers to Saaremaa and Dobrava hantaviruses , and five showed the highest endpoint titers to Puumala hantavirus .
	manualset3
221487	1	420672	7	NULL	NULL	0	NULL	formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation of macrophage-derived foam cells in a plaque is a hallmark of the development of atherosclerosis .
	manualset3
221488	2	420672	7	NULL	NULL	0	NULL	macrophage-derived foam cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation of macrophage-derived foam cells in a plaque is a hallmark of the development of atherosclerosis .
	manualset3
221489	3	420672	7	NULL	NULL	0	NULL	plaque	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation of macrophage-derived foam cells in a plaque is a hallmark of the development of atherosclerosis .
	manualset3
221490	4	420672	7	NULL	NULL	0	NULL	 hallmark	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation of macrophage-derived foam cells in a plaque is a hallmark of the development of atherosclerosis .
	manualset3
221491	5	420672	7	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation of macrophage-derived foam cells in a plaque is a hallmark of the development of atherosclerosis .
	manualset3
221492	6	420672	7	NULL	NULL	0	NULL	atherosclerosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation of macrophage-derived foam cells in a plaque is a hallmark of the development of atherosclerosis .
	manualset3
221493	1	420673	7	NULL	NULL	0	NULL	Cytotoxic T cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Cytotoxic T cells play a critical role in the control of HIV and the progression of infected individuals to AIDS .
	manualset3
221494	2	420673	7	NULL	NULL	NULL	NULL	critical role	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytotoxic T cells play a critical role in the control of HIV and the progression of infected individuals to AIDS .
	manualset3
221495	3	420673	7	NULL	NULL	0	NULL	control	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cytotoxic T cells play a critical role in the control of HIV and the progression of infected individuals to AIDS .
	manualset3
221496	4	420673	7	NULL	NULL	0	NULL	HIV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Cytotoxic T cells play a critical role in the control of HIV and the progression of infected individuals to AIDS .
	manualset3
221497	5	420673	7	NULL	NULL	0	NULL	progression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cytotoxic T cells play a critical role in the control of HIV and the progression of infected individuals to AIDS .
	manualset3
221498	6	420673	7	NULL	NULL	0	NULL	infected individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Cytotoxic T cells play a critical role in the control of HIV and the progression of infected individuals to AIDS .
	manualset3
221499	7	420673	7	NULL	NULL	0	NULL	AIDS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Cytotoxic T cells play a critical role in the control of HIV and the progression of infected individuals to AIDS .
	manualset3
221500	1	420674	7	NULL	NULL	NULL	NULL	Chromosomal damage	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Chromosomal damage was evaluated by means of the cytokinesis block micronucleus technique , which also gives information on cell cycle kinetics .
	manualset3
221501	2	420674	7	NULL	NULL	0	NULL	cytokinesis block micronucleus technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Chromosomal damage was evaluated by means of the cytokinesis block micronucleus technique , which also gives information on cell cycle kinetics .
	manualset3
221502	3	420674	7	NULL	NULL	0	NULL	information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Chromosomal damage was evaluated by means of the cytokinesis block micronucleus technique , which also gives information on cell cycle kinetics .
	manualset3
221503	4	420674	7	NULL	NULL	0	NULL	cell cycle kinetics 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Chromosomal damage was evaluated by means of the cytokinesis block micronucleus technique , which also gives information on cell cycle kinetics .
	manualset3
221504	1	420675	7	NULL	NULL	0	NULL	Immunoreactivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoreactivity for beta-endorphin in LH-RH neurons of the fetal human hypothalamus .
	manualset3
221505	2	420675	7	NULL	NULL	0	NULL	beta-endorphin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoreactivity for beta-endorphin in LH-RH neurons of the fetal human hypothalamus .
	manualset3
221506	3	420675	7	NULL	NULL	0	NULL	LH-RH neurons	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoreactivity for beta-endorphin in LH-RH neurons of the fetal human hypothalamus .
	manualset3
221507	4	420675	7	NULL	NULL	0	NULL	 fetal human hypothalamus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoreactivity for beta-endorphin in LH-RH neurons of the fetal human hypothalamus .
	manualset3
221508	1	420676	7	NULL	NULL	0	NULL	Final revision	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Final revision to OMB circular A-110 .
	manualset3
221509	2	420676	7	NULL	NULL	0	NULL	OMB circular A-110	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Final revision to OMB circular A-110 .
	manualset3
221510	1	420677	7	NULL	NULL	0	NULL	models 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These models enable us to manipulate rationally the properties of enzymes , here to design an `` acetaldehyde reductase '' dependent on NAD + that is faster than any given us by nature .
	manualset3
221511	2	420677	7	NULL	NULL	0	NULL	properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These models enable us to manipulate rationally the properties of enzymes , here to design an `` acetaldehyde reductase '' dependent on NAD + that is faster than any given us by nature .
	manualset3
221512	3	420677	7	NULL	NULL	0	NULL	enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These models enable us to manipulate rationally the properties of enzymes , here to design an `` acetaldehyde reductase '' dependent on NAD + that is faster than any given us by nature .
	manualset3
221513	4	420677	7	NULL	NULL	0	NULL	acetaldehyde reductase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These models enable us to manipulate rationally the properties of enzymes , here to design an `` acetaldehyde reductase '' dependent on NAD + that is faster than any given us by nature .
	manualset3
221514	5	420677	7	NULL	NULL	0	NULL	NAD +	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These models enable us to manipulate rationally the properties of enzymes , here to design an `` acetaldehyde reductase '' dependent on NAD + that is faster than any given us by nature .
	manualset3
221515	6	420677	7	NULL	NULL	0	NULL	nature	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These models enable us to manipulate rationally the properties of enzymes , here to design an `` acetaldehyde reductase '' dependent on NAD + that is faster than any given us by nature .
	manualset3
221516	1	420678	7	NULL	NULL	0	NULL	New directions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	New directions in nursing education .
	manualset3
221517	2	420678	7	NULL	NULL	0	NULL	nursing education	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	New directions in nursing education .
	manualset3
221518	1	420679	7	NULL	NULL	0	NULL	meal-induced secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A meal-induced secretion appears to be the most sensitive to the inhibitory action of intraduodenal somatostatin , probably because of the suppression of gastric acid and serum gastrin secretin involved in the postprandial stimulation of the exocrine pancreas .
	manualset3
221519	2	420679	7	NULL	NULL	0	NULL	inhibitory action	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A meal-induced secretion appears to be the most sensitive to the inhibitory action of intraduodenal somatostatin , probably because of the suppression of gastric acid and serum gastrin secretin involved in the postprandial stimulation of the exocrine pancreas .
	manualset3
221520	3	420679	7	NULL	NULL	0	NULL	intraduodenal somatostatin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A meal-induced secretion appears to be the most sensitive to the inhibitory action of intraduodenal somatostatin , probably because of the suppression of gastric acid and serum gastrin secretin involved in the postprandial stimulation of the exocrine pancreas .
	manualset3
221521	4	420679	7	NULL	NULL	0	NULL	suppression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A meal-induced secretion appears to be the most sensitive to the inhibitory action of intraduodenal somatostatin , probably because of the suppression of gastric acid and serum gastrin secretin involved in the postprandial stimulation of the exocrine pancreas .
	manualset3
221522	5	420679	7	NULL	NULL	0	NULL	gastric acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A meal-induced secretion appears to be the most sensitive to the inhibitory action of intraduodenal somatostatin , probably because of the suppression of gastric acid and serum gastrin secretin involved in the postprandial stimulation of the exocrine pancreas .
	manualset3
221523	6	420679	7	NULL	NULL	0	NULL	serum gastrin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A meal-induced secretion appears to be the most sensitive to the inhibitory action of intraduodenal somatostatin , probably because of the suppression of gastric acid and serum gastrin secretin involved in the postprandial stimulation of the exocrine pancreas .
	manualset3
221524	7	420679	7	NULL	NULL	0	NULL	secretin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A meal-induced secretion appears to be the most sensitive to the inhibitory action of intraduodenal somatostatin , probably because of the suppression of gastric acid and serum gastrin secretin involved in the postprandial stimulation of the exocrine pancreas .
	manualset3
221525	8	420679	7	NULL	NULL	0	NULL	 postprandial stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A meal-induced secretion appears to be the most sensitive to the inhibitory action of intraduodenal somatostatin , probably because of the suppression of gastric acid and serum gastrin secretin involved in the postprandial stimulation of the exocrine pancreas .
	manualset3
221526	9	420679	7	NULL	NULL	0	NULL	exocrine pancreas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A meal-induced secretion appears to be the most sensitive to the inhibitory action of intraduodenal somatostatin , probably because of the suppression of gastric acid and serum gastrin secretin involved in the postprandial stimulation of the exocrine pancreas .
	manualset3
221527	1	420680	7	NULL	NULL	0	NULL	small region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Only a small region , centered on area V3A and extending into V4 and DPL , contained cells labeled by either injection as well as a small number of double-labeled cells .
	manualset3
221528	2	420680	7	NULL	NULL	0	NULL	area V3A 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Only a small region , centered on area V3A and extending into V4 and DPL , contained cells labeled by either injection as well as a small number of double-labeled cells .
	manualset3
221529	3	420680	7	NULL	NULL	0	NULL	V4	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Only a small region , centered on area V3A and extending into V4 and DPL , contained cells labeled by either injection as well as a small number of double-labeled cells .
	manualset3
221530	4	420680	7	NULL	NULL	0	NULL	DPL	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Only a small region , centered on area V3A and extending into V4 and DPL , contained cells labeled by either injection as well as a small number of double-labeled cells .
	manualset3
221531	5	420680	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Only a small region , centered on area V3A and extending into V4 and DPL , contained cells labeled by either injection as well as a small number of double-labeled cells .
	manualset3
221532	6	420680	7	NULL	NULL	0	NULL	 injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Only a small region , centered on area V3A and extending into V4 and DPL , contained cells labeled by either injection as well as a small number of double-labeled cells .
	manualset3
221533	7	420680	7	NULL	NULL	0	NULL	small number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Only a small region , centered on area V3A and extending into V4 and DPL , contained cells labeled by either injection as well as a small number of double-labeled cells .
	manualset3
221534	8	420680	7	NULL	NULL	0	NULL	double-labeled cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Only a small region , centered on area V3A and extending into V4 and DPL , contained cells labeled by either injection as well as a small number of double-labeled cells .
	manualset3
221535	1	420681	7	NULL	NULL	0	NULL	3961 infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 3961 infants checked at the ages of 3 -- 7 days and again at 6 weeks 42 % showed nevi flammei mediales in the nape and/or in the eyelids and glabella .
	manualset3
221536	2	420681	7	NULL	NULL	0	NULL	ages	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 3961 infants checked at the ages of 3 -- 7 days and again at 6 weeks 42 % showed nevi flammei mediales in the nape and/or in the eyelids and glabella .
	manualset3
221537	3	420681	7	NULL	NULL	0	NULL	3 -- 7 days 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 3961 infants checked at the ages of 3 -- 7 days and again at 6 weeks 42 % showed nevi flammei mediales in the nape and/or in the eyelids and glabella .
	manualset3
221538	4	420681	7	NULL	NULL	0	NULL	6 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 3961 infants checked at the ages of 3 -- 7 days and again at 6 weeks 42 % showed nevi flammei mediales in the nape and/or in the eyelids and glabella .
	manualset3
221539	5	420681	7	NULL	NULL	0	NULL	42 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 3961 infants checked at the ages of 3 -- 7 days and again at 6 weeks 42 % showed nevi flammei mediales in the nape and/or in the eyelids and glabella .
	manualset3
221540	6	420681	7	NULL	NULL	0	NULL	nevi flammei mediales	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 3961 infants checked at the ages of 3 -- 7 days and again at 6 weeks 42 % showed nevi flammei mediales in the nape and/or in the eyelids and glabella .
	manualset3
221541	7	420681	7	NULL	NULL	0	NULL	nape	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 3961 infants checked at the ages of 3 -- 7 days and again at 6 weeks 42 % showed nevi flammei mediales in the nape and/or in the eyelids and glabella .
	manualset3
221542	8	420681	7	NULL	NULL	0	NULL	eyelids	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 3961 infants checked at the ages of 3 -- 7 days and again at 6 weeks 42 % showed nevi flammei mediales in the nape and/or in the eyelids and glabella .
	manualset3
221543	9	420681	7	NULL	NULL	0	NULL	glabella	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 3961 infants checked at the ages of 3 -- 7 days and again at 6 weeks 42 % showed nevi flammei mediales in the nape and/or in the eyelids and glabella .
	manualset3
221544	1	420682	7	NULL	NULL	0	NULL	Two cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of hamartoangiomyomatosis with characteristic scintigraphic findings .
	manualset3
221545	2	420682	7	NULL	NULL	0	NULL	hamartoangiomyomatosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of hamartoangiomyomatosis with characteristic scintigraphic findings .
	manualset3
221546	3	420682	7	NULL	NULL	0	NULL	scintigraphic findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two cases of hamartoangiomyomatosis with characteristic scintigraphic findings .
	manualset3
221547	1	420683	7	NULL	NULL	0	NULL	benefit of gestures 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The benefit of gestures persists even in subsequent spatial visualization problems in which gesture is prohibited .
	manualset3
221548	2	420683	7	NULL	NULL	0	NULL	spatial visualization problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The benefit of gestures persists even in subsequent spatial visualization problems in which gesture is prohibited .
	manualset3
221549	3	420683	7	NULL	NULL	0	NULL	 gesture	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The benefit of gestures persists even in subsequent spatial visualization problems in which gesture is prohibited .
	manualset3
221550	1	420684	7	NULL	NULL	0	NULL	Chambers	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Chambers containing VEGF ( 500-700 ng/ml ) in a laminin-based gel ( Matrigel ) were inserted into 1 cm rat sciatic nerve defects and nerve regeneration examined in relation to angiogenesis between 5 and 180 d. Longitudinal sections were stained with antibodies against endothelial cells ( RECA-1 ) , axons ( neurofilament ) and Schwann cells ( S-100 ) to follow the progression of vascular and neural elements .
	manualset3
221551	2	420684	7	NULL	NULL	0	NULL	VEGF 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Chambers containing VEGF ( 500-700 ng/ml ) in a laminin-based gel ( Matrigel ) were inserted into 1 cm rat sciatic nerve defects and nerve regeneration examined in relation to angiogenesis between 5 and 180 d. Longitudinal sections were stained with antibodies against endothelial cells ( RECA-1 ) , axons ( neurofilament ) and Schwann cells ( S-100 ) to follow the progression of vascular and neural elements .
	manualset3
221552	3	420684	7	NULL	NULL	0	NULL	500-700 ng/ml	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Chambers containing VEGF ( 500-700 ng/ml ) in a laminin-based gel ( Matrigel ) were inserted into 1 cm rat sciatic nerve defects and nerve regeneration examined in relation to angiogenesis between 5 and 180 d. Longitudinal sections were stained with antibodies against endothelial cells ( RECA-1 ) , axons ( neurofilament ) and Schwann cells ( S-100 ) to follow the progression of vascular and neural elements .
	manualset3
221553	4	420684	7	NULL	NULL	0	NULL	laminin-based gel ( Matrigel )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Chambers containing VEGF ( 500-700 ng/ml ) in a laminin-based gel ( Matrigel ) were inserted into 1 cm rat sciatic nerve defects and nerve regeneration examined in relation to angiogenesis between 5 and 180 d. Longitudinal sections were stained with antibodies against endothelial cells ( RECA-1 ) , axons ( neurofilament ) and Schwann cells ( S-100 ) to follow the progression of vascular and neural elements .
	manualset3
221554	5	420684	7	NULL	NULL	0	NULL	1 cm rat sciatic nerve defects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Chambers containing VEGF ( 500-700 ng/ml ) in a laminin-based gel ( Matrigel ) were inserted into 1 cm rat sciatic nerve defects and nerve regeneration examined in relation to angiogenesis between 5 and 180 d. Longitudinal sections were stained with antibodies against endothelial cells ( RECA-1 ) , axons ( neurofilament ) and Schwann cells ( S-100 ) to follow the progression of vascular and neural elements .
	manualset3
221555	6	420684	7	NULL	NULL	0	NULL	nerve regeneration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Chambers containing VEGF ( 500-700 ng/ml ) in a laminin-based gel ( Matrigel ) were inserted into 1 cm rat sciatic nerve defects and nerve regeneration examined in relation to angiogenesis between 5 and 180 d. Longitudinal sections were stained with antibodies against endothelial cells ( RECA-1 ) , axons ( neurofilament ) and Schwann cells ( S-100 ) to follow the progression of vascular and neural elements .
	manualset3
221556	7	420684	7	NULL	NULL	0	NULL	angiogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Chambers containing VEGF ( 500-700 ng/ml ) in a laminin-based gel ( Matrigel ) were inserted into 1 cm rat sciatic nerve defects and nerve regeneration examined in relation to angiogenesis between 5 and 180 d. Longitudinal sections were stained with antibodies against endothelial cells ( RECA-1 ) , axons ( neurofilament ) and Schwann cells ( S-100 ) to follow the progression of vascular and neural elements .
	manualset3
221557	8	420684	7	NULL	NULL	0	NULL	5 d	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Chambers containing VEGF ( 500-700 ng/ml ) in a laminin-based gel ( Matrigel ) were inserted into 1 cm rat sciatic nerve defects and nerve regeneration examined in relation to angiogenesis between 5 and 180 d. Longitudinal sections were stained with antibodies against endothelial cells ( RECA-1 ) , axons ( neurofilament ) and Schwann cells ( S-100 ) to follow the progression of vascular and neural elements .
	manualset3
221558	9	420684	7	NULL	NULL	0	NULL	180 d	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Chambers containing VEGF ( 500-700 ng/ml ) in a laminin-based gel ( Matrigel ) were inserted into 1 cm rat sciatic nerve defects and nerve regeneration examined in relation to angiogenesis between 5 and 180 d. Longitudinal sections were stained with antibodies against endothelial cells ( RECA-1 ) , axons ( neurofilament ) and Schwann cells ( S-100 ) to follow the progression of vascular and neural elements .
	manualset3
221559	10	420684	7	NULL	NULL	0	NULL	Longitudinal sections	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Chambers containing VEGF ( 500-700 ng/ml ) in a laminin-based gel ( Matrigel ) were inserted into 1 cm rat sciatic nerve defects and nerve regeneration examined in relation to angiogenesis between 5 and 180 d. Longitudinal sections were stained with antibodies against endothelial cells ( RECA-1 ) , axons ( neurofilament ) and Schwann cells ( S-100 ) to follow the progression of vascular and neural elements .
	manualset3
221560	11	420684	7	NULL	NULL	0	NULL	antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Chambers containing VEGF ( 500-700 ng/ml ) in a laminin-based gel ( Matrigel ) were inserted into 1 cm rat sciatic nerve defects and nerve regeneration examined in relation to angiogenesis between 5 and 180 d. Longitudinal sections were stained with antibodies against endothelial cells ( RECA-1 ) , axons ( neurofilament ) and Schwann cells ( S-100 ) to follow the progression of vascular and neural elements .
	manualset3
221561	12	420684	7	NULL	NULL	0	NULL	endothelial cells ( RECA-1 )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Chambers containing VEGF ( 500-700 ng/ml ) in a laminin-based gel ( Matrigel ) were inserted into 1 cm rat sciatic nerve defects and nerve regeneration examined in relation to angiogenesis between 5 and 180 d. Longitudinal sections were stained with antibodies against endothelial cells ( RECA-1 ) , axons ( neurofilament ) and Schwann cells ( S-100 ) to follow the progression of vascular and neural elements .
	manualset3
221562	13	420684	7	NULL	NULL	0	NULL	axons ( neurofilament )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Chambers containing VEGF ( 500-700 ng/ml ) in a laminin-based gel ( Matrigel ) were inserted into 1 cm rat sciatic nerve defects and nerve regeneration examined in relation to angiogenesis between 5 and 180 d. Longitudinal sections were stained with antibodies against endothelial cells ( RECA-1 ) , axons ( neurofilament ) and Schwann cells ( S-100 ) to follow the progression of vascular and neural elements .
	manualset3
221563	14	420684	7	NULL	NULL	0	NULL	Schwann cells ( S-100 )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Chambers containing VEGF ( 500-700 ng/ml ) in a laminin-based gel ( Matrigel ) were inserted into 1 cm rat sciatic nerve defects and nerve regeneration examined in relation to angiogenesis between 5 and 180 d. Longitudinal sections were stained with antibodies against endothelial cells ( RECA-1 ) , axons ( neurofilament ) and Schwann cells ( S-100 ) to follow the progression of vascular and neural elements .
	manualset3
221564	15	420684	7	NULL	NULL	0	NULL	progression 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Chambers containing VEGF ( 500-700 ng/ml ) in a laminin-based gel ( Matrigel ) were inserted into 1 cm rat sciatic nerve defects and nerve regeneration examined in relation to angiogenesis between 5 and 180 d. Longitudinal sections were stained with antibodies against endothelial cells ( RECA-1 ) , axons ( neurofilament ) and Schwann cells ( S-100 ) to follow the progression of vascular and neural elements .
	manualset3
221565	16	420684	7	NULL	NULL	NULL	NULL	vascular elements	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Chambers containing VEGF ( 500-700 ng/ml ) in a laminin-based gel ( Matrigel ) were inserted into 1 cm rat sciatic nerve defects and nerve regeneration examined in relation to angiogenesis between 5 and 180 d. Longitudinal sections were stained with antibodies against endothelial cells ( RECA-1 ) , axons ( neurofilament ) and Schwann cells ( S-100 ) to follow the progression of vascular and neural elements .
	manualset3
221566	17	420684	7	NULL	NULL	NULL	NULL	neural elements	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Chambers containing VEGF ( 500-700 ng/ml ) in a laminin-based gel ( Matrigel ) were inserted into 1 cm rat sciatic nerve defects and nerve regeneration examined in relation to angiogenesis between 5 and 180 d. Longitudinal sections were stained with antibodies against endothelial cells ( RECA-1 ) , axons ( neurofilament ) and Schwann cells ( S-100 ) to follow the progression of vascular and neural elements .
	manualset3
223244	18	420684	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Chambers containing VEGF ( 500-700 ng/ml ) in a laminin-based gel ( Matrigel ) were inserted into 1 cm rat sciatic nerve defects and nerve regeneration examined in relation to angiogenesis between 5 and 180 d. Longitudinal sections were stained with antibodies against endothelial cells ( RECA-1 ) , axons ( neurofilament ) and Schwann cells ( S-100 ) to follow the progression of vascular and neural elements .
	manualset3
221567	1	420685	7	NULL	NULL	0	NULL	hematological neoplasms CD56 ( N-CAM )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In hematological neoplasms CD56 ( N-CAM ) is expressed by T/natural killer ( NK ) cell lymphoma , by most neoplastic plasma cells in multiple myeloma and also in a subset of acute myelogenous leukemias ( AML ) .
	manualset3
221568	2	420685	7	NULL	NULL	0	NULL	T/natural killer ( NK ) cell lymphoma	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In hematological neoplasms CD56 ( N-CAM ) is expressed by T/natural killer ( NK ) cell lymphoma , by most neoplastic plasma cells in multiple myeloma and also in a subset of acute myelogenous leukemias ( AML ) .
	manualset3
221569	3	420685	7	NULL	NULL	0	NULL	neoplastic plasma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In hematological neoplasms CD56 ( N-CAM ) is expressed by T/natural killer ( NK ) cell lymphoma , by most neoplastic plasma cells in multiple myeloma and also in a subset of acute myelogenous leukemias ( AML ) .
	manualset3
221570	4	420685	7	NULL	NULL	0	NULL	multiple myeloma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In hematological neoplasms CD56 ( N-CAM ) is expressed by T/natural killer ( NK ) cell lymphoma , by most neoplastic plasma cells in multiple myeloma and also in a subset of acute myelogenous leukemias ( AML ) .
	manualset3
221571	5	420685	7	NULL	NULL	0	NULL	subset of acute myelogenous leukemias ( AML ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In hematological neoplasms CD56 ( N-CAM ) is expressed by T/natural killer ( NK ) cell lymphoma , by most neoplastic plasma cells in multiple myeloma and also in a subset of acute myelogenous leukemias ( AML ) .
	manualset3
221572	1	420686	7	NULL	NULL	0	NULL	methods	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Our methods demonstrate the feasibility of using ANN to develop individualized wheelchair tilt and recline guidance for people with SCI .
	manualset3
221573	2	420686	7	NULL	NULL	0	NULL	feasibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our methods demonstrate the feasibility of using ANN to develop individualized wheelchair tilt and recline guidance for people with SCI .
	manualset3
221574	3	420686	7	NULL	NULL	0	NULL	 ANN	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Our methods demonstrate the feasibility of using ANN to develop individualized wheelchair tilt and recline guidance for people with SCI .
	manualset3
221575	4	420686	7	NULL	NULL	0	NULL	wheelchair tilt	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Our methods demonstrate the feasibility of using ANN to develop individualized wheelchair tilt and recline guidance for people with SCI .
	manualset3
221576	5	420686	7	NULL	NULL	0	NULL	 recline guidance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our methods demonstrate the feasibility of using ANN to develop individualized wheelchair tilt and recline guidance for people with SCI .
	manualset3
221577	6	420686	7	NULL	NULL	0	NULL	people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our methods demonstrate the feasibility of using ANN to develop individualized wheelchair tilt and recline guidance for people with SCI .
	manualset3
221578	7	420686	7	NULL	NULL	0	NULL	SCI	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our methods demonstrate the feasibility of using ANN to develop individualized wheelchair tilt and recline guidance for people with SCI .
	manualset3
221579	1	420687	7	NULL	NULL	0	NULL	Racial variations 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Racial variations in postoperative outcomes of carotid endarterectomy : evidence from the Veterans Affairs National Surgical Quality Improvement Program .
	manualset3
221580	2	420687	7	NULL	NULL	0	NULL	postoperative outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Racial variations in postoperative outcomes of carotid endarterectomy : evidence from the Veterans Affairs National Surgical Quality Improvement Program .
	manualset3
221581	3	420687	7	NULL	NULL	0	NULL	carotid endarterectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Racial variations in postoperative outcomes of carotid endarterectomy : evidence from the Veterans Affairs National Surgical Quality Improvement Program .
	manualset3
221582	4	420687	7	NULL	NULL	0	NULL	 evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Racial variations in postoperative outcomes of carotid endarterectomy : evidence from the Veterans Affairs National Surgical Quality Improvement Program .
	manualset3
221583	5	420687	7	NULL	NULL	0	NULL	Veterans Affairs National Surgical Quality Improvement Program	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Racial variations in postoperative outcomes of carotid endarterectomy : evidence from the Veterans Affairs National Surgical Quality Improvement Program .
	manualset3
221584	1	420688	7	NULL	NULL	0	NULL	Angiotensin II AT1 receptor signal transduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin II AT1 receptor signal transduction has recently been shown to function through the phospholipase C isozyme , PLC-gamma .
	manualset3
221585	2	420688	7	NULL	NULL	0	NULL	phospholipase C isozyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin II AT1 receptor signal transduction has recently been shown to function through the phospholipase C isozyme , PLC-gamma .
	manualset3
221586	3	420688	7	NULL	NULL	0	NULL	 PLC-gamma	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin II AT1 receptor signal transduction has recently been shown to function through the phospholipase C isozyme , PLC-gamma .
	manualset3
221587	1	420689	7	NULL	NULL	0	NULL	45 clinic personnel 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 45 clinic personnel , 16 reported recent skin infections , and 4 % were colonized with MRSA .
	manualset3
221588	2	420689	7	NULL	NULL	0	NULL	16	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 45 clinic personnel , 16 reported recent skin infections , and 4 % were colonized with MRSA .
	manualset3
221589	3	420689	7	NULL	NULL	0	NULL	skin infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 45 clinic personnel , 16 reported recent skin infections , and 4 % were colonized with MRSA .
	manualset3
221590	4	420689	7	NULL	NULL	0	NULL	4 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 45 clinic personnel , 16 reported recent skin infections , and 4 % were colonized with MRSA .
	manualset3
221591	5	420689	7	NULL	NULL	0	NULL	MRSA	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 45 clinic personnel , 16 reported recent skin infections , and 4 % were colonized with MRSA .
	manualset3
221592	1	420690	7	NULL	NULL	0	NULL	Two patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients developed de novo hepatitis B infection and two required additional HBIG injections .
	manualset3
221593	2	420690	7	NULL	NULL	0	NULL	de novo hepatitis B infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients developed de novo hepatitis B infection and two required additional HBIG injections .
	manualset3
221594	3	420690	7	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients developed de novo hepatitis B infection and two required additional HBIG injections .
	manualset3
221595	4	420690	7	NULL	NULL	0	NULL	HBIG injections	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Two patients developed de novo hepatitis B infection and two required additional HBIG injections .
	manualset3
221596	1	420691	7	NULL	NULL	0	NULL	slopes	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The slopes of the individual growth trajectories , the graphic representations of rates of progress , were comparable in the eight children .
	manualset3
221597	2	420691	7	NULL	NULL	0	NULL	individual growth trajectories	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The slopes of the individual growth trajectories , the graphic representations of rates of progress , were comparable in the eight children .
	manualset3
221598	3	420691	7	NULL	NULL	0	NULL	graphic representations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The slopes of the individual growth trajectories , the graphic representations of rates of progress , were comparable in the eight children .
	manualset3
221599	4	420691	7	NULL	NULL	0	NULL	rates of progress	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The slopes of the individual growth trajectories , the graphic representations of rates of progress , were comparable in the eight children .
	manualset3
221600	5	420691	7	NULL	NULL	0	NULL	eight children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The slopes of the individual growth trajectories , the graphic representations of rates of progress , were comparable in the eight children .
	manualset3
221601	1	420692	7	NULL	NULL	0	NULL	human ribonuclease ( RNase )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we discovered that human ribonuclease ( RNase ) , deoxyribonuclease I ( DNase I ) and deoxyribonuclease II ( DNase II ) are characteristic markers showing genetic polymorphism and useful for forensic investigation .
	manualset3
221602	2	420692	7	NULL	NULL	0	NULL	deoxyribonuclease I ( DNase I )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we discovered that human ribonuclease ( RNase ) , deoxyribonuclease I ( DNase I ) and deoxyribonuclease II ( DNase II ) are characteristic markers showing genetic polymorphism and useful for forensic investigation .
	manualset3
221603	3	420692	7	NULL	NULL	0	NULL	deoxyribonuclease II ( DNase II )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we discovered that human ribonuclease ( RNase ) , deoxyribonuclease I ( DNase I ) and deoxyribonuclease II ( DNase II ) are characteristic markers showing genetic polymorphism and useful for forensic investigation .
	manualset3
221604	4	420692	7	NULL	NULL	0	NULL	markers	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we discovered that human ribonuclease ( RNase ) , deoxyribonuclease I ( DNase I ) and deoxyribonuclease II ( DNase II ) are characteristic markers showing genetic polymorphism and useful for forensic investigation .
	manualset3
221605	5	420692	7	NULL	NULL	0	NULL	genetic polymorphism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we discovered that human ribonuclease ( RNase ) , deoxyribonuclease I ( DNase I ) and deoxyribonuclease II ( DNase II ) are characteristic markers showing genetic polymorphism and useful for forensic investigation .
	manualset3
221606	6	420692	7	NULL	NULL	0	NULL	forensic investigation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently , we discovered that human ribonuclease ( RNase ) , deoxyribonuclease I ( DNase I ) and deoxyribonuclease II ( DNase II ) are characteristic markers showing genetic polymorphism and useful for forensic investigation .
	manualset3
221607	1	420693	7	NULL	NULL	0	NULL	gonadotropin stimulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we have recently discovered that gonadotropin stimulation can activate the MAPK cascade in target cells .
	manualset3
221608	2	420693	7	NULL	NULL	0	NULL	MAPK cascade 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we have recently discovered that gonadotropin stimulation can activate the MAPK cascade in target cells .
	manualset3
221609	3	420693	7	NULL	NULL	0	NULL	target cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we have recently discovered that gonadotropin stimulation can activate the MAPK cascade in target cells .
	manualset3
221610	1	420694	7	NULL	NULL	0	NULL	stroke	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The stroke has only a minor influence on direction consistency in golf putting among elite players .
	manualset3
221611	2	420694	7	NULL	NULL	0	NULL	minor influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The stroke has only a minor influence on direction consistency in golf putting among elite players .
	manualset3
221612	3	420694	7	NULL	NULL	0	NULL	direction consistency	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The stroke has only a minor influence on direction consistency in golf putting among elite players .
	manualset3
221613	4	420694	7	NULL	NULL	0	NULL	golf	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The stroke has only a minor influence on direction consistency in golf putting among elite players .
	manualset3
221614	5	420694	7	NULL	NULL	0	NULL	elite players	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The stroke has only a minor influence on direction consistency in golf putting among elite players .
	manualset3
221615	1	420695	7	NULL	NULL	0	NULL	Induction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of Id3 is accomplished by angiotensin II via superoxide release .
	manualset3
221616	2	420695	7	NULL	NULL	0	NULL	Id3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of Id3 is accomplished by angiotensin II via superoxide release .
	manualset3
221617	3	420695	7	NULL	NULL	0	NULL	angiotensin II 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of Id3 is accomplished by angiotensin II via superoxide release .
	manualset3
221618	4	420695	7	NULL	NULL	0	NULL	superoxide release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of Id3 is accomplished by angiotensin II via superoxide release .
	manualset3
221619	1	420696	7	NULL	NULL	0	NULL	Anterior palatal fistulae	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Anterior palatal fistulae immediately behind the incisor teeth may be difficult to repair .
	manualset3
221620	2	420696	7	NULL	NULL	0	NULL	incisor teeth	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Anterior palatal fistulae immediately behind the incisor teeth may be difficult to repair .
	manualset3
221621	3	420696	7	NULL	NULL	0	NULL	repair	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Anterior palatal fistulae immediately behind the incisor teeth may be difficult to repair .
	manualset3
221622	1	420697	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that pentobarbital and muscimol may induce feeding by acting on a similar hypothalamic receptor complex but by different mechanisms .
	manualset3
221623	2	420697	7	NULL	NULL	0	NULL	pentobarbital	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that pentobarbital and muscimol may induce feeding by acting on a similar hypothalamic receptor complex but by different mechanisms .
	manualset3
221624	3	420697	7	NULL	NULL	0	NULL	muscimol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that pentobarbital and muscimol may induce feeding by acting on a similar hypothalamic receptor complex but by different mechanisms .
	manualset3
221625	4	420697	7	NULL	NULL	NULL	NULL	feeding	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The data suggest that pentobarbital and muscimol may induce feeding by acting on a similar hypothalamic receptor complex but by different mechanisms .
	manualset3
221626	5	420697	7	NULL	NULL	0	NULL	hypothalamic receptor complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that pentobarbital and muscimol may induce feeding by acting on a similar hypothalamic receptor complex but by different mechanisms .
	manualset3
221627	6	420697	7	NULL	NULL	0	NULL	different mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The data suggest that pentobarbital and muscimol may induce feeding by acting on a similar hypothalamic receptor complex but by different mechanisms .
	manualset3
221628	1	420698	7	NULL	NULL	0	NULL	over-expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , over-expression of UCP2 was also found in leukemia , ovarian , bladder , esophagus , testicular , colorectal , kidney , pancreatic , lung and prostate tumors .
	manualset3
221629	2	420698	7	NULL	NULL	0	NULL	UCP2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , over-expression of UCP2 was also found in leukemia , ovarian , bladder , esophagus , testicular , colorectal , kidney , pancreatic , lung and prostate tumors .
	manualset3
221630	3	420698	7	NULL	NULL	0	NULL	leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , over-expression of UCP2 was also found in leukemia , ovarian , bladder , esophagus , testicular , colorectal , kidney , pancreatic , lung and prostate tumors .
	manualset3
221631	4	420698	7	NULL	NULL	0	NULL	ovarian tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , over-expression of UCP2 was also found in leukemia , ovarian , bladder , esophagus , testicular , colorectal , kidney , pancreatic , lung and prostate tumors .
	manualset3
221632	5	420698	7	NULL	NULL	0	NULL	bladder tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , over-expression of UCP2 was also found in leukemia , ovarian , bladder , esophagus , testicular , colorectal , kidney , pancreatic , lung and prostate tumors .
	manualset3
221633	6	420698	7	NULL	NULL	0	NULL	 esophagus tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , over-expression of UCP2 was also found in leukemia , ovarian , bladder , esophagus , testicular , colorectal , kidney , pancreatic , lung and prostate tumors .
	manualset3
221634	7	420698	7	NULL	NULL	0	NULL	testicular tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , over-expression of UCP2 was also found in leukemia , ovarian , bladder , esophagus , testicular , colorectal , kidney , pancreatic , lung and prostate tumors .
	manualset3
221635	8	420698	7	NULL	NULL	0	NULL	 colorectal tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , over-expression of UCP2 was also found in leukemia , ovarian , bladder , esophagus , testicular , colorectal , kidney , pancreatic , lung and prostate tumors .
	manualset3
221636	9	420698	7	NULL	NULL	0	NULL	kidney tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , over-expression of UCP2 was also found in leukemia , ovarian , bladder , esophagus , testicular , colorectal , kidney , pancreatic , lung and prostate tumors .
	manualset3
221637	10	420698	7	NULL	NULL	0	NULL	pancreatic tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , over-expression of UCP2 was also found in leukemia , ovarian , bladder , esophagus , testicular , colorectal , kidney , pancreatic , lung and prostate tumors .
	manualset3
221638	11	420698	7	NULL	NULL	0	NULL	 lung tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , over-expression of UCP2 was also found in leukemia , ovarian , bladder , esophagus , testicular , colorectal , kidney , pancreatic , lung and prostate tumors .
	manualset3
221639	12	420698	7	NULL	NULL	0	NULL	prostate tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , over-expression of UCP2 was also found in leukemia , ovarian , bladder , esophagus , testicular , colorectal , kidney , pancreatic , lung and prostate tumors .
	manualset3
221640	1	420699	7	NULL	NULL	0	NULL	 multiple occlusions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The same applies to multiple occlusions in the same vein meaning that venous occlusions in the deep veins of the lower limb can not be examined separately .
	manualset3
221641	2	420699	7	NULL	NULL	0	NULL	same vein	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The same applies to multiple occlusions in the same vein meaning that venous occlusions in the deep veins of the lower limb can not be examined separately .
	manualset3
221642	3	420699	7	NULL	NULL	0	NULL	venous occlusions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The same applies to multiple occlusions in the same vein meaning that venous occlusions in the deep veins of the lower limb can not be examined separately .
	manualset3
221643	4	420699	7	NULL	NULL	0	NULL	deep veins of the lower limb	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The same applies to multiple occlusions in the same vein meaning that venous occlusions in the deep veins of the lower limb can not be examined separately .
	manualset3
221644	5	420699	7	NULL	NULL	0	NULL	lower limb	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The same applies to multiple occlusions in the same vein meaning that venous occlusions in the deep veins of the lower limb can not be examined separately .
	manualset3
221645	1	420700	7	NULL	NULL	NULL	NULL	Ten transplant patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ten transplant patients receiving a liposomal amphotericin B formulation ( AmBisome ) were compared to ten retrospective control patients given conventional amphotericin B. Each group included bone marrow ( 8 ) , kidney ( 1 ) , and liver transplant ( 1 ) recipients .
	manualset3
221646	2	420700	7	NULL	NULL	0	NULL	liposomal amphotericin B formulation ( AmBisome )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten transplant patients receiving a liposomal amphotericin B formulation ( AmBisome ) were compared to ten retrospective control patients given conventional amphotericin B. Each group included bone marrow ( 8 ) , kidney ( 1 ) , and liver transplant ( 1 ) recipients .
	manualset3
221647	3	420700	7	NULL	NULL	0	NULL	ten	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten transplant patients receiving a liposomal amphotericin B formulation ( AmBisome ) were compared to ten retrospective control patients given conventional amphotericin B. Each group included bone marrow ( 8 ) , kidney ( 1 ) , and liver transplant ( 1 ) recipients .
	manualset3
221648	4	420700	7	NULL	NULL	0	NULL	retrospective control patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten transplant patients receiving a liposomal amphotericin B formulation ( AmBisome ) were compared to ten retrospective control patients given conventional amphotericin B. Each group included bone marrow ( 8 ) , kidney ( 1 ) , and liver transplant ( 1 ) recipients .
	manualset3
221649	5	420700	7	NULL	NULL	0	NULL	conventional amphotericin B	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten transplant patients receiving a liposomal amphotericin B formulation ( AmBisome ) were compared to ten retrospective control patients given conventional amphotericin B. Each group included bone marrow ( 8 ) , kidney ( 1 ) , and liver transplant ( 1 ) recipients .
	manualset3
221650	6	420700	7	NULL	NULL	0	NULL	 group 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten transplant patients receiving a liposomal amphotericin B formulation ( AmBisome ) were compared to ten retrospective control patients given conventional amphotericin B. Each group included bone marrow ( 8 ) , kidney ( 1 ) , and liver transplant ( 1 ) recipients .
	manualset3
221651	7	420700	7	NULL	NULL	0	NULL	bone marrow	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten transplant patients receiving a liposomal amphotericin B formulation ( AmBisome ) were compared to ten retrospective control patients given conventional amphotericin B. Each group included bone marrow ( 8 ) , kidney ( 1 ) , and liver transplant ( 1 ) recipients .
	manualset3
221652	8	420700	7	NULL	NULL	0	NULL	8	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten transplant patients receiving a liposomal amphotericin B formulation ( AmBisome ) were compared to ten retrospective control patients given conventional amphotericin B. Each group included bone marrow ( 8 ) , kidney ( 1 ) , and liver transplant ( 1 ) recipients .
	manualset3
221653	9	420700	7	NULL	NULL	0	NULL	kidney	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten transplant patients receiving a liposomal amphotericin B formulation ( AmBisome ) were compared to ten retrospective control patients given conventional amphotericin B. Each group included bone marrow ( 8 ) , kidney ( 1 ) , and liver transplant ( 1 ) recipients .
	manualset3
221654	10	420700	7	NULL	NULL	0	NULL	1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten transplant patients receiving a liposomal amphotericin B formulation ( AmBisome ) were compared to ten retrospective control patients given conventional amphotericin B. Each group included bone marrow ( 8 ) , kidney ( 1 ) , and liver transplant ( 1 ) recipients .
	manualset3
221655	11	420700	7	NULL	NULL	0	NULL	liver transplant recipients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten transplant patients receiving a liposomal amphotericin B formulation ( AmBisome ) were compared to ten retrospective control patients given conventional amphotericin B. Each group included bone marrow ( 8 ) , kidney ( 1 ) , and liver transplant ( 1 ) recipients .
	manualset3
221656	12	420700	7	NULL	NULL	0	NULL	1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ten transplant patients receiving a liposomal amphotericin B formulation ( AmBisome ) were compared to ten retrospective control patients given conventional amphotericin B. Each group included bone marrow ( 8 ) , kidney ( 1 ) , and liver transplant ( 1 ) recipients .
	manualset3
221657	1	420701	7	NULL	NULL	0	NULL	enzymatically active organellar form	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Besides the enzymatically active organellar form of acyl-CoA oxidase , the monomeric apoprotein was detected when short-term labeling of cotyledons in vivo was performed .
	manualset3
221658	2	420701	7	NULL	NULL	0	NULL	acyl-CoA oxidase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Besides the enzymatically active organellar form of acyl-CoA oxidase , the monomeric apoprotein was detected when short-term labeling of cotyledons in vivo was performed .
	manualset3
221659	3	420701	7	NULL	NULL	0	NULL	monomeric apoprotein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Besides the enzymatically active organellar form of acyl-CoA oxidase , the monomeric apoprotein was detected when short-term labeling of cotyledons in vivo was performed .
	manualset3
221660	4	420701	7	NULL	NULL	0	NULL	short-term labeling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Besides the enzymatically active organellar form of acyl-CoA oxidase , the monomeric apoprotein was detected when short-term labeling of cotyledons in vivo was performed .
	manualset3
221661	5	420701	7	NULL	NULL	0	NULL	cotyledons	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Besides the enzymatically active organellar form of acyl-CoA oxidase , the monomeric apoprotein was detected when short-term labeling of cotyledons in vivo was performed .
	manualset3
221662	1	420702	7	NULL	NULL	0	NULL	Synovial fluid examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Synovial fluid examination with polarized microscopy was initially negative , but revealed numerous CPPD crystals when repeated on the third hospital day .
	manualset3
221663	2	420702	7	NULL	NULL	0	NULL	polarized microscopy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Synovial fluid examination with polarized microscopy was initially negative , but revealed numerous CPPD crystals when repeated on the third hospital day .
	manualset3
221664	3	420702	7	NULL	NULL	0	NULL	numerous CPPD crystals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Synovial fluid examination with polarized microscopy was initially negative , but revealed numerous CPPD crystals when repeated on the third hospital day .
	manualset3
221665	4	420702	7	NULL	NULL	0	NULL	third hospital day 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Synovial fluid examination with polarized microscopy was initially negative , but revealed numerous CPPD crystals when repeated on the third hospital day .
	manualset3
221666	1	420703	7	NULL	NULL	0	NULL	 EMs	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among EMs , debrisoquine MR was significantly ( P & lt ; 0.05 ) lower during smoking cessation ( mean antilog + / - SD , 0.48 + / - 0.29 ) compared to a smoking period ( 0.61 + / - 0.23 ) .
	manualset3
221667	2	420703	7	NULL	NULL	0	NULL	debrisoquine MR	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Among EMs , debrisoquine MR was significantly ( P & lt ; 0.05 ) lower during smoking cessation ( mean antilog + / - SD , 0.48 + / - 0.29 ) compared to a smoking period ( 0.61 + / - 0.23 ) .
	manualset3
221668	3	420703	7	NULL	NULL	0	NULL	P & lt ; 0.05	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among EMs , debrisoquine MR was significantly ( P & lt ; 0.05 ) lower during smoking cessation ( mean antilog + / - SD , 0.48 + / - 0.29 ) compared to a smoking period ( 0.61 + / - 0.23 ) .
	manualset3
221669	4	420703	7	NULL	NULL	0	NULL	smoking cessation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among EMs , debrisoquine MR was significantly ( P & lt ; 0.05 ) lower during smoking cessation ( mean antilog + / - SD , 0.48 + / - 0.29 ) compared to a smoking period ( 0.61 + / - 0.23 ) .
	manualset3
221670	5	420703	7	NULL	NULL	0	NULL	mean antilog 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among EMs , debrisoquine MR was significantly ( P & lt ; 0.05 ) lower during smoking cessation ( mean antilog + / - SD , 0.48 + / - 0.29 ) compared to a smoking period ( 0.61 + / - 0.23 ) .
	manualset3
221671	6	420703	7	NULL	NULL	0	NULL	+ / - SD , 0.48 + / - 0.29 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among EMs , debrisoquine MR was significantly ( P & lt ; 0.05 ) lower during smoking cessation ( mean antilog + / - SD , 0.48 + / - 0.29 ) compared to a smoking period ( 0.61 + / - 0.23 ) .
	manualset3
221672	7	420703	7	NULL	NULL	0	NULL	smoking period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Among EMs , debrisoquine MR was significantly ( P & lt ; 0.05 ) lower during smoking cessation ( mean antilog + / - SD , 0.48 + / - 0.29 ) compared to a smoking period ( 0.61 + / - 0.23 ) .
	manualset3
221673	8	420703	7	NULL	NULL	0	NULL	0.61 + / - 0.23	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among EMs , debrisoquine MR was significantly ( P & lt ; 0.05 ) lower during smoking cessation ( mean antilog + / - SD , 0.48 + / - 0.29 ) compared to a smoking period ( 0.61 + / - 0.23 ) .
	manualset3
221674	1	420704	7	NULL	NULL	0	NULL	Pure naproxen particles 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Pure naproxen particles and mixed naproxen-polylactic acid particles were formed by pulsed rapid expansion of supercritical CO2 solutions ( RESS ) .
	manualset3
221675	2	420704	7	NULL	NULL	0	NULL	mixed naproxen-polylactic acid particles	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Pure naproxen particles and mixed naproxen-polylactic acid particles were formed by pulsed rapid expansion of supercritical CO2 solutions ( RESS ) .
	manualset3
221676	3	420704	7	NULL	NULL	NULL	NULL	pulsed rapid expansion of supercritical CO2 solutions ( RESS )	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pure naproxen particles and mixed naproxen-polylactic acid particles were formed by pulsed rapid expansion of supercritical CO2 solutions ( RESS ) .
	manualset3
221677	1	420705	7	NULL	NULL	0	NULL	 efficacy 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of a single dose of teicoplanin ( 18 mg/kg of body weight given intramuscularly ) for the prevention of endocarditis due to Streptococcus oralis , Enterococcus faecium , and methicillin-resistant Staphylococcus aureus ( MRSA ) was evaluated after applying the rabbit model .
	manualset3
221678	2	420705	7	NULL	NULL	0	NULL	single dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of a single dose of teicoplanin ( 18 mg/kg of body weight given intramuscularly ) for the prevention of endocarditis due to Streptococcus oralis , Enterococcus faecium , and methicillin-resistant Staphylococcus aureus ( MRSA ) was evaluated after applying the rabbit model .
	manualset3
221679	3	420705	7	NULL	NULL	0	NULL	teicoplanin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of a single dose of teicoplanin ( 18 mg/kg of body weight given intramuscularly ) for the prevention of endocarditis due to Streptococcus oralis , Enterococcus faecium , and methicillin-resistant Staphylococcus aureus ( MRSA ) was evaluated after applying the rabbit model .
	manualset3
221680	4	420705	7	NULL	NULL	0	NULL	18 mg/kg of body weight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of a single dose of teicoplanin ( 18 mg/kg of body weight given intramuscularly ) for the prevention of endocarditis due to Streptococcus oralis , Enterococcus faecium , and methicillin-resistant Staphylococcus aureus ( MRSA ) was evaluated after applying the rabbit model .
	manualset3
221681	5	420705	7	NULL	NULL	0	NULL	prevention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of a single dose of teicoplanin ( 18 mg/kg of body weight given intramuscularly ) for the prevention of endocarditis due to Streptococcus oralis , Enterococcus faecium , and methicillin-resistant Staphylococcus aureus ( MRSA ) was evaluated after applying the rabbit model .
	manualset3
221682	6	420705	7	NULL	NULL	0	NULL	endocarditis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of a single dose of teicoplanin ( 18 mg/kg of body weight given intramuscularly ) for the prevention of endocarditis due to Streptococcus oralis , Enterococcus faecium , and methicillin-resistant Staphylococcus aureus ( MRSA ) was evaluated after applying the rabbit model .
	manualset3
221683	7	420705	7	NULL	NULL	0	NULL	Streptococcus oralis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of a single dose of teicoplanin ( 18 mg/kg of body weight given intramuscularly ) for the prevention of endocarditis due to Streptococcus oralis , Enterococcus faecium , and methicillin-resistant Staphylococcus aureus ( MRSA ) was evaluated after applying the rabbit model .
	manualset3
221684	8	420705	7	NULL	NULL	0	NULL	Enterococcus faecium	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of a single dose of teicoplanin ( 18 mg/kg of body weight given intramuscularly ) for the prevention of endocarditis due to Streptococcus oralis , Enterococcus faecium , and methicillin-resistant Staphylococcus aureus ( MRSA ) was evaluated after applying the rabbit model .
	manualset3
221685	9	420705	7	NULL	NULL	0	NULL	methicillin-resistant Staphylococcus aureus ( MRSA )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of a single dose of teicoplanin ( 18 mg/kg of body weight given intramuscularly ) for the prevention of endocarditis due to Streptococcus oralis , Enterococcus faecium , and methicillin-resistant Staphylococcus aureus ( MRSA ) was evaluated after applying the rabbit model .
	manualset3
221686	10	420705	7	NULL	NULL	0	NULL	 rabbit model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The efficacy of a single dose of teicoplanin ( 18 mg/kg of body weight given intramuscularly ) for the prevention of endocarditis due to Streptococcus oralis , Enterococcus faecium , and methicillin-resistant Staphylococcus aureus ( MRSA ) was evaluated after applying the rabbit model .
	manualset3
221687	1	420706	7	NULL	NULL	0	NULL	OP pesticides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	OP pesticides are metabolized to dialkylphosphates and other metabolites , which are excreted in urine .
	manualset3
221688	2	420706	7	NULL	NULL	0	NULL	dialkylphosphates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	OP pesticides are metabolized to dialkylphosphates and other metabolites , which are excreted in urine .
	manualset3
221689	3	420706	7	NULL	NULL	0	NULL	metabolites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	OP pesticides are metabolized to dialkylphosphates and other metabolites , which are excreted in urine .
	manualset3
221690	4	420706	7	NULL	NULL	0	NULL	urine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	OP pesticides are metabolized to dialkylphosphates and other metabolites , which are excreted in urine .
	manualset3
221691	1	420707	7	NULL	NULL	0	NULL	condition	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a condition has been attributed to the fact that the filler particles are held to the surface of the resin matrix primarily by mechanical means .
	manualset3
221692	2	420707	7	NULL	NULL	0	NULL	 filler particles	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a condition has been attributed to the fact that the filler particles are held to the surface of the resin matrix primarily by mechanical means .
	manualset3
221693	3	420707	7	NULL	NULL	0	NULL	surface	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a condition has been attributed to the fact that the filler particles are held to the surface of the resin matrix primarily by mechanical means .
	manualset3
221694	4	420707	7	NULL	NULL	0	NULL	resin matrix	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Such a condition has been attributed to the fact that the filler particles are held to the surface of the resin matrix primarily by mechanical means .
	manualset3
221695	1	420708	7	NULL	NULL	0	NULL	Fluorescein-conjugated WGA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescein-conjugated WGA was demonstrated to transport from the cell surface into the paranuclear region of cultured L929 cells within 30 min , and subsequently evoked lipid peroxidation of plasma membrane and vacuolation in the cytoplasm of these cells .
	manualset3
221696	2	420708	7	NULL	NULL	0	NULL	 cell surface	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescein-conjugated WGA was demonstrated to transport from the cell surface into the paranuclear region of cultured L929 cells within 30 min , and subsequently evoked lipid peroxidation of plasma membrane and vacuolation in the cytoplasm of these cells .
	manualset3
221697	3	420708	7	NULL	NULL	0	NULL	 paranuclear region 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescein-conjugated WGA was demonstrated to transport from the cell surface into the paranuclear region of cultured L929 cells within 30 min , and subsequently evoked lipid peroxidation of plasma membrane and vacuolation in the cytoplasm of these cells .
	manualset3
221698	4	420708	7	NULL	NULL	0	NULL	cultured L929 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescein-conjugated WGA was demonstrated to transport from the cell surface into the paranuclear region of cultured L929 cells within 30 min , and subsequently evoked lipid peroxidation of plasma membrane and vacuolation in the cytoplasm of these cells .
	manualset3
221699	5	420708	7	NULL	NULL	0	NULL	30 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescein-conjugated WGA was demonstrated to transport from the cell surface into the paranuclear region of cultured L929 cells within 30 min , and subsequently evoked lipid peroxidation of plasma membrane and vacuolation in the cytoplasm of these cells .
	manualset3
221700	6	420708	7	NULL	NULL	0	NULL	lipid peroxidation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescein-conjugated WGA was demonstrated to transport from the cell surface into the paranuclear region of cultured L929 cells within 30 min , and subsequently evoked lipid peroxidation of plasma membrane and vacuolation in the cytoplasm of these cells .
	manualset3
221701	7	420708	7	NULL	NULL	0	NULL	plasma membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescein-conjugated WGA was demonstrated to transport from the cell surface into the paranuclear region of cultured L929 cells within 30 min , and subsequently evoked lipid peroxidation of plasma membrane and vacuolation in the cytoplasm of these cells .
	manualset3
221702	8	420708	7	NULL	NULL	NULL	NULL	vacuolation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fluorescein-conjugated WGA was demonstrated to transport from the cell surface into the paranuclear region of cultured L929 cells within 30 min , and subsequently evoked lipid peroxidation of plasma membrane and vacuolation in the cytoplasm of these cells .
	manualset3
221703	9	420708	7	NULL	NULL	0	NULL	cytoplasm 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescein-conjugated WGA was demonstrated to transport from the cell surface into the paranuclear region of cultured L929 cells within 30 min , and subsequently evoked lipid peroxidation of plasma membrane and vacuolation in the cytoplasm of these cells .
	manualset3
221704	10	420708	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescein-conjugated WGA was demonstrated to transport from the cell surface into the paranuclear region of cultured L929 cells within 30 min , and subsequently evoked lipid peroxidation of plasma membrane and vacuolation in the cytoplasm of these cells .
	manualset3
221705	1	420709	7	NULL	NULL	0	NULL	intestinal bacteria 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It is well known that some intestinal bacteria , such as Escherichia coli , can produce a remarkable amount of molecular hydrogen ( H ( 2 ) ) .
	manualset3
221706	2	420709	7	NULL	NULL	0	NULL	Escherichia coli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It is well known that some intestinal bacteria , such as Escherichia coli , can produce a remarkable amount of molecular hydrogen ( H ( 2 ) ) .
	manualset3
221707	3	420709	7	NULL	NULL	0	NULL	remarkable amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It is well known that some intestinal bacteria , such as Escherichia coli , can produce a remarkable amount of molecular hydrogen ( H ( 2 ) ) .
	manualset3
221708	4	420709	7	NULL	NULL	0	NULL	molecular hydrogen ( H ( 2 ) )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is well known that some intestinal bacteria , such as Escherichia coli , can produce a remarkable amount of molecular hydrogen ( H ( 2 ) ) .
	manualset3
221709	1	420710	7	NULL	NULL	0	NULL	Mean values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean values for PM10 in indoor climbing halls are generally on the order of 200-500 microg m ( -3 ) .
	manualset3
221710	2	420710	7	NULL	NULL	0	NULL	 PM10	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean values for PM10 in indoor climbing halls are generally on the order of 200-500 microg m ( -3 ) .
	manualset3
221711	3	420710	7	NULL	NULL	0	NULL	indoor climbing halls 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean values for PM10 in indoor climbing halls are generally on the order of 200-500 microg m ( -3 ) .
	manualset3
221712	4	420710	7	NULL	NULL	0	NULL	 order	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean values for PM10 in indoor climbing halls are generally on the order of 200-500 microg m ( -3 ) .
	manualset3
221713	5	420710	7	NULL	NULL	0	NULL	200-500 microg m ( -3 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean values for PM10 in indoor climbing halls are generally on the order of 200-500 microg m ( -3 ) .
	manualset3
221714	1	420711	7	NULL	NULL	0	NULL	antigen-immunized mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among antigen-immunized mice , NP-reactive GC B cell populations in the antigen-induced GC consisted mostly of cells expressing the canonical V186 .2 gene which contained , on average , 0.8 point mutations/V ( H ) gene by day 8 after immunization .
	manualset3
221715	2	420711	7	NULL	NULL	0	NULL	NP-reactive GC B cell populations	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Among antigen-immunized mice , NP-reactive GC B cell populations in the antigen-induced GC consisted mostly of cells expressing the canonical V186 .2 gene which contained , on average , 0.8 point mutations/V ( H ) gene by day 8 after immunization .
	manualset3
221716	3	420711	7	NULL	NULL	0	NULL	antigen-induced GC	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Among antigen-immunized mice , NP-reactive GC B cell populations in the antigen-induced GC consisted mostly of cells expressing the canonical V186 .2 gene which contained , on average , 0.8 point mutations/V ( H ) gene by day 8 after immunization .
	manualset3
221717	4	420711	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Among antigen-immunized mice , NP-reactive GC B cell populations in the antigen-induced GC consisted mostly of cells expressing the canonical V186 .2 gene which contained , on average , 0.8 point mutations/V ( H ) gene by day 8 after immunization .
	manualset3
221718	5	420711	7	NULL	NULL	0	NULL	canonical V186 .2 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Among antigen-immunized mice , NP-reactive GC B cell populations in the antigen-induced GC consisted mostly of cells expressing the canonical V186 .2 gene which contained , on average , 0.8 point mutations/V ( H ) gene by day 8 after immunization .
	manualset3
221719	6	420711	7	NULL	NULL	0	NULL	average	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among antigen-immunized mice , NP-reactive GC B cell populations in the antigen-induced GC consisted mostly of cells expressing the canonical V186 .2 gene which contained , on average , 0.8 point mutations/V ( H ) gene by day 8 after immunization .
	manualset3
221720	7	420711	7	NULL	NULL	0	NULL	0.8 point mutations/V ( H ) gene	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among antigen-immunized mice , NP-reactive GC B cell populations in the antigen-induced GC consisted mostly of cells expressing the canonical V186 .2 gene which contained , on average , 0.8 point mutations/V ( H ) gene by day 8 after immunization .
	manualset3
221721	8	420711	7	NULL	NULL	0	NULL	day 8 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Among antigen-immunized mice , NP-reactive GC B cell populations in the antigen-induced GC consisted mostly of cells expressing the canonical V186 .2 gene which contained , on average , 0.8 point mutations/V ( H ) gene by day 8 after immunization .
	manualset3
221722	9	420711	7	NULL	NULL	0	NULL	 immunization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among antigen-immunized mice , NP-reactive GC B cell populations in the antigen-induced GC consisted mostly of cells expressing the canonical V186 .2 gene which contained , on average , 0.8 point mutations/V ( H ) gene by day 8 after immunization .
	manualset3
221723	1	420712	7	NULL	NULL	0	NULL	insensitivities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the insensitivities of generic MAU measures in COPD can lead to biased cost-effectiveness analyses and ill-informed economic decisions .
	manualset3
221724	2	420712	7	NULL	NULL	0	NULL	generic MAU measures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the insensitivities of generic MAU measures in COPD can lead to biased cost-effectiveness analyses and ill-informed economic decisions .
	manualset3
221725	3	420712	7	NULL	NULL	0	NULL	COPD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the insensitivities of generic MAU measures in COPD can lead to biased cost-effectiveness analyses and ill-informed economic decisions .
	manualset3
221726	4	420712	7	NULL	NULL	0	NULL	biased cost-effectiveness analyses 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the insensitivities of generic MAU measures in COPD can lead to biased cost-effectiveness analyses and ill-informed economic decisions .
	manualset3
221727	5	420712	7	NULL	NULL	0	NULL	ill-informed economic decisions	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Overall , the insensitivities of generic MAU measures in COPD can lead to biased cost-effectiveness analyses and ill-informed economic decisions .
	manualset3
221728	1	420713	7	NULL	NULL	0	NULL	T3S substrate specificity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	T3S substrate specificity is controlled by the cytoplasmic switch protein HpaC , which interacts with the C-terminal domain of the inner membrane protein HrcU ( HrcU ( C ) ) .
	manualset3
221729	2	420713	7	NULL	NULL	0	NULL	cytoplasmic switch protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	T3S substrate specificity is controlled by the cytoplasmic switch protein HpaC , which interacts with the C-terminal domain of the inner membrane protein HrcU ( HrcU ( C ) ) .
	manualset3
221730	3	420713	7	NULL	NULL	0	NULL	HpaC	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	T3S substrate specificity is controlled by the cytoplasmic switch protein HpaC , which interacts with the C-terminal domain of the inner membrane protein HrcU ( HrcU ( C ) ) .
	manualset3
221731	4	420713	7	NULL	NULL	0	NULL	C-terminal domain 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	T3S substrate specificity is controlled by the cytoplasmic switch protein HpaC , which interacts with the C-terminal domain of the inner membrane protein HrcU ( HrcU ( C ) ) .
	manualset3
221732	5	420713	7	NULL	NULL	0	NULL	 inner membrane protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	T3S substrate specificity is controlled by the cytoplasmic switch protein HpaC , which interacts with the C-terminal domain of the inner membrane protein HrcU ( HrcU ( C ) ) .
	manualset3
221733	6	420713	7	NULL	NULL	0	NULL	HrcU ( HrcU ( C ) )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	T3S substrate specificity is controlled by the cytoplasmic switch protein HpaC , which interacts with the C-terminal domain of the inner membrane protein HrcU ( HrcU ( C ) ) .
	manualset3
221734	1	420714	7	NULL	NULL	0	NULL	specificity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( The specificity of liver arginase and of intestinal heteroarginase .
	manualset3
221735	2	420714	7	NULL	NULL	0	NULL	liver arginase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( The specificity of liver arginase and of intestinal heteroarginase .
	manualset3
221736	3	420714	7	NULL	NULL	0	NULL	intestinal heteroarginase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( The specificity of liver arginase and of intestinal heteroarginase .
	manualset3
221737	1	420715	7	NULL	NULL	0	NULL	22-year old man	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A 22-year old man was admitted to the emergency room of our hospital with bleeding from scrotal wound .
	manualset3
221738	2	420715	7	NULL	NULL	0	NULL	emergency room	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A 22-year old man was admitted to the emergency room of our hospital with bleeding from scrotal wound .
	manualset3
221739	3	420715	7	NULL	NULL	0	NULL	hospital	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A 22-year old man was admitted to the emergency room of our hospital with bleeding from scrotal wound .
	manualset3
221740	4	420715	7	NULL	NULL	0	NULL	bleeding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 22-year old man was admitted to the emergency room of our hospital with bleeding from scrotal wound .
	manualset3
221741	5	420715	7	NULL	NULL	0	NULL	scrotal wound	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 22-year old man was admitted to the emergency room of our hospital with bleeding from scrotal wound .
	manualset3
221742	1	420716	7	NULL	NULL	0	NULL	Sequence similarity	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence similarity with a stretch of amino acids involved in the receptor-binding pocket of the influenza A hemagglutinin suggests that the mutation site on the influenza C glycoprotein ( HEF ) is part of the receptor-binding site .
	manualset3
221743	2	420716	7	NULL	NULL	0	NULL	stretch of amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence similarity with a stretch of amino acids involved in the receptor-binding pocket of the influenza A hemagglutinin suggests that the mutation site on the influenza C glycoprotein ( HEF ) is part of the receptor-binding site .
	manualset3
221744	3	420716	7	NULL	NULL	0	NULL	receptor-binding pocket	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence similarity with a stretch of amino acids involved in the receptor-binding pocket of the influenza A hemagglutinin suggests that the mutation site on the influenza C glycoprotein ( HEF ) is part of the receptor-binding site .
	manualset3
221745	4	420716	7	NULL	NULL	0	NULL	influenza A hemagglutinin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence similarity with a stretch of amino acids involved in the receptor-binding pocket of the influenza A hemagglutinin suggests that the mutation site on the influenza C glycoprotein ( HEF ) is part of the receptor-binding site .
	manualset3
221746	5	420716	7	NULL	NULL	0	NULL	mutation site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence similarity with a stretch of amino acids involved in the receptor-binding pocket of the influenza A hemagglutinin suggests that the mutation site on the influenza C glycoprotein ( HEF ) is part of the receptor-binding site .
	manualset3
221747	6	420716	7	NULL	NULL	0	NULL	 influenza C glycoprotein ( HEF ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence similarity with a stretch of amino acids involved in the receptor-binding pocket of the influenza A hemagglutinin suggests that the mutation site on the influenza C glycoprotein ( HEF ) is part of the receptor-binding site .
	manualset3
221748	7	420716	7	NULL	NULL	0	NULL	receptor-binding site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence similarity with a stretch of amino acids involved in the receptor-binding pocket of the influenza A hemagglutinin suggests that the mutation site on the influenza C glycoprotein ( HEF ) is part of the receptor-binding site .
	manualset3
221749	1	420717	7	NULL	NULL	0	NULL	Adjuvant therapies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Adjuvant therapies for patients with melanoma at high risk of relapse whether local , such as excision margins , elective regional lymph node dissection ( ELND ) , and prophylactic isolated limb perfusion ( ILP ) , or systemic , such as chemotherapy , immunotherapy , immunochemotherapy , or vaccination therapy , have little or no impact on survival when evaluated in randomized trials .
	manualset3
221750	2	420717	7	NULL	NULL	0	NULL	 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Adjuvant therapies for patients with melanoma at high risk of relapse whether local , such as excision margins , elective regional lymph node dissection ( ELND ) , and prophylactic isolated limb perfusion ( ILP ) , or systemic , such as chemotherapy , immunotherapy , immunochemotherapy , or vaccination therapy , have little or no impact on survival when evaluated in randomized trials .
	manualset3
221751	3	420717	7	NULL	NULL	0	NULL	melanoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Adjuvant therapies for patients with melanoma at high risk of relapse whether local , such as excision margins , elective regional lymph node dissection ( ELND ) , and prophylactic isolated limb perfusion ( ILP ) , or systemic , such as chemotherapy , immunotherapy , immunochemotherapy , or vaccination therapy , have little or no impact on survival when evaluated in randomized trials .
	manualset3
221752	4	420717	7	NULL	NULL	0	NULL	high risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Adjuvant therapies for patients with melanoma at high risk of relapse whether local , such as excision margins , elective regional lymph node dissection ( ELND ) , and prophylactic isolated limb perfusion ( ILP ) , or systemic , such as chemotherapy , immunotherapy , immunochemotherapy , or vaccination therapy , have little or no impact on survival when evaluated in randomized trials .
	manualset3
221753	5	420717	7	NULL	NULL	0	NULL	relapse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Adjuvant therapies for patients with melanoma at high risk of relapse whether local , such as excision margins , elective regional lymph node dissection ( ELND ) , and prophylactic isolated limb perfusion ( ILP ) , or systemic , such as chemotherapy , immunotherapy , immunochemotherapy , or vaccination therapy , have little or no impact on survival when evaluated in randomized trials .
	manualset3
221754	6	420717	7	NULL	NULL	0	NULL	excision margins	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Adjuvant therapies for patients with melanoma at high risk of relapse whether local , such as excision margins , elective regional lymph node dissection ( ELND ) , and prophylactic isolated limb perfusion ( ILP ) , or systemic , such as chemotherapy , immunotherapy , immunochemotherapy , or vaccination therapy , have little or no impact on survival when evaluated in randomized trials .
	manualset3
221755	7	420717	7	NULL	NULL	0	NULL	elective regional lymph node dissection ( ELND ) 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Adjuvant therapies for patients with melanoma at high risk of relapse whether local , such as excision margins , elective regional lymph node dissection ( ELND ) , and prophylactic isolated limb perfusion ( ILP ) , or systemic , such as chemotherapy , immunotherapy , immunochemotherapy , or vaccination therapy , have little or no impact on survival when evaluated in randomized trials .
	manualset3
221756	8	420717	7	NULL	NULL	0	NULL	prophylactic isolated limb perfusion ( ILP ) 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Adjuvant therapies for patients with melanoma at high risk of relapse whether local , such as excision margins , elective regional lymph node dissection ( ELND ) , and prophylactic isolated limb perfusion ( ILP ) , or systemic , such as chemotherapy , immunotherapy , immunochemotherapy , or vaccination therapy , have little or no impact on survival when evaluated in randomized trials .
	manualset3
221757	9	420717	7	NULL	NULL	0	NULL	chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Adjuvant therapies for patients with melanoma at high risk of relapse whether local , such as excision margins , elective regional lymph node dissection ( ELND ) , and prophylactic isolated limb perfusion ( ILP ) , or systemic , such as chemotherapy , immunotherapy , immunochemotherapy , or vaccination therapy , have little or no impact on survival when evaluated in randomized trials .
	manualset3
221758	10	420717	7	NULL	NULL	0	NULL	immunotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Adjuvant therapies for patients with melanoma at high risk of relapse whether local , such as excision margins , elective regional lymph node dissection ( ELND ) , and prophylactic isolated limb perfusion ( ILP ) , or systemic , such as chemotherapy , immunotherapy , immunochemotherapy , or vaccination therapy , have little or no impact on survival when evaluated in randomized trials .
	manualset3
221759	11	420717	7	NULL	NULL	0	NULL	 immunochemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Adjuvant therapies for patients with melanoma at high risk of relapse whether local , such as excision margins , elective regional lymph node dissection ( ELND ) , and prophylactic isolated limb perfusion ( ILP ) , or systemic , such as chemotherapy , immunotherapy , immunochemotherapy , or vaccination therapy , have little or no impact on survival when evaluated in randomized trials .
	manualset3
221760	12	420717	7	NULL	NULL	0	NULL	vaccination therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Adjuvant therapies for patients with melanoma at high risk of relapse whether local , such as excision margins , elective regional lymph node dissection ( ELND ) , and prophylactic isolated limb perfusion ( ILP ) , or systemic , such as chemotherapy , immunotherapy , immunochemotherapy , or vaccination therapy , have little or no impact on survival when evaluated in randomized trials .
	manualset3
221761	13	420717	7	NULL	NULL	0	NULL	survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Adjuvant therapies for patients with melanoma at high risk of relapse whether local , such as excision margins , elective regional lymph node dissection ( ELND ) , and prophylactic isolated limb perfusion ( ILP ) , or systemic , such as chemotherapy , immunotherapy , immunochemotherapy , or vaccination therapy , have little or no impact on survival when evaluated in randomized trials .
	manualset3
221762	14	420717	7	NULL	NULL	0	NULL	randomized trials	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Adjuvant therapies for patients with melanoma at high risk of relapse whether local , such as excision margins , elective regional lymph node dissection ( ELND ) , and prophylactic isolated limb perfusion ( ILP ) , or systemic , such as chemotherapy , immunotherapy , immunochemotherapy , or vaccination therapy , have little or no impact on survival when evaluated in randomized trials .
	manualset3
221763	1	420718	7	NULL	NULL	0	NULL	M. chelonei strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( iii ) All M. chelonei and M. fortuitum strains survived 60 min of exposure to concentrations of 0.3 and 0.7 microgram of free chlorine per ml at pH 7 .
	manualset3
221764	2	420718	7	NULL	NULL	0	NULL	 M. fortuitum strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( iii ) All M. chelonei and M. fortuitum strains survived 60 min of exposure to concentrations of 0.3 and 0.7 microgram of free chlorine per ml at pH 7 .
	manualset3
221765	3	420718	7	NULL	NULL	0	NULL	60 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	( iii ) All M. chelonei and M. fortuitum strains survived 60 min of exposure to concentrations of 0.3 and 0.7 microgram of free chlorine per ml at pH 7 .
	manualset3
221766	4	420718	7	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( iii ) All M. chelonei and M. fortuitum strains survived 60 min of exposure to concentrations of 0.3 and 0.7 microgram of free chlorine per ml at pH 7 .
	manualset3
221767	5	420718	7	NULL	NULL	0	NULL	concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( iii ) All M. chelonei and M. fortuitum strains survived 60 min of exposure to concentrations of 0.3 and 0.7 microgram of free chlorine per ml at pH 7 .
	manualset3
221768	6	420718	7	NULL	NULL	0	NULL	0.3 microgram 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( iii ) All M. chelonei and M. fortuitum strains survived 60 min of exposure to concentrations of 0.3 and 0.7 microgram of free chlorine per ml at pH 7 .
	manualset3
221769	7	420718	7	NULL	NULL	0	NULL	 0.7 microgram	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( iii ) All M. chelonei and M. fortuitum strains survived 60 min of exposure to concentrations of 0.3 and 0.7 microgram of free chlorine per ml at pH 7 .
	manualset3
221770	8	420718	7	NULL	NULL	NULL	NULL	free chlorine per ml	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( iii ) All M. chelonei and M. fortuitum strains survived 60 min of exposure to concentrations of 0.3 and 0.7 microgram of free chlorine per ml at pH 7 .
	manualset3
221771	9	420718	7	NULL	NULL	0	NULL	pH 7	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( iii ) All M. chelonei and M. fortuitum strains survived 60 min of exposure to concentrations of 0.3 and 0.7 microgram of free chlorine per ml at pH 7 .
	manualset3
221772	1	420719	7	NULL	NULL	0	NULL	cancer samples 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Among cancer samples , larger increases in choline , and decreases in citrate and polyamines ( P = 0.05 ) were observed with more aggressive cancers , and a MIB-1 labeling index correlated ( r = 0.62 , P = 0.01 ) with elevated choline .
	manualset3
221773	2	420719	7	NULL	NULL	0	NULL	choline	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Among cancer samples , larger increases in choline , and decreases in citrate and polyamines ( P = 0.05 ) were observed with more aggressive cancers , and a MIB-1 labeling index correlated ( r = 0.62 , P = 0.01 ) with elevated choline .
	manualset3
221774	3	420719	7	NULL	NULL	0	NULL	citrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Among cancer samples , larger increases in choline , and decreases in citrate and polyamines ( P = 0.05 ) were observed with more aggressive cancers , and a MIB-1 labeling index correlated ( r = 0.62 , P = 0.01 ) with elevated choline .
	manualset3
221775	4	420719	7	NULL	NULL	0	NULL	polyamines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Among cancer samples , larger increases in choline , and decreases in citrate and polyamines ( P = 0.05 ) were observed with more aggressive cancers , and a MIB-1 labeling index correlated ( r = 0.62 , P = 0.01 ) with elevated choline .
	manualset3
221776	5	420719	7	NULL	NULL	0	NULL	P = 0.05	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among cancer samples , larger increases in choline , and decreases in citrate and polyamines ( P = 0.05 ) were observed with more aggressive cancers , and a MIB-1 labeling index correlated ( r = 0.62 , P = 0.01 ) with elevated choline .
	manualset3
221777	6	420719	7	NULL	NULL	0	NULL	aggressive cancers	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Among cancer samples , larger increases in choline , and decreases in citrate and polyamines ( P = 0.05 ) were observed with more aggressive cancers , and a MIB-1 labeling index correlated ( r = 0.62 , P = 0.01 ) with elevated choline .
	manualset3
221778	7	420719	7	NULL	NULL	0	NULL	MIB-1 labeling index	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among cancer samples , larger increases in choline , and decreases in citrate and polyamines ( P = 0.05 ) were observed with more aggressive cancers , and a MIB-1 labeling index correlated ( r = 0.62 , P = 0.01 ) with elevated choline .
	manualset3
221779	8	420719	7	NULL	NULL	0	NULL	r = 0.62	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among cancer samples , larger increases in choline , and decreases in citrate and polyamines ( P = 0.05 ) were observed with more aggressive cancers , and a MIB-1 labeling index correlated ( r = 0.62 , P = 0.01 ) with elevated choline .
	manualset3
221780	9	420719	7	NULL	NULL	0	NULL	P = 0.01 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among cancer samples , larger increases in choline , and decreases in citrate and polyamines ( P = 0.05 ) were observed with more aggressive cancers , and a MIB-1 labeling index correlated ( r = 0.62 , P = 0.01 ) with elevated choline .
	manualset3
221781	10	420719	7	NULL	NULL	0	NULL	elevated choline	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among cancer samples , larger increases in choline , and decreases in citrate and polyamines ( P = 0.05 ) were observed with more aggressive cancers , and a MIB-1 labeling index correlated ( r = 0.62 , P = 0.01 ) with elevated choline .
	manualset3
221782	1	420720	7	NULL	NULL	0	NULL	Mammalian sirtuin 1 ( SIRT1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mammalian sirtuin 1 ( SIRT1 ) may control fatty acid homeostasis in liver .
	manualset3
221783	2	420720	7	NULL	NULL	0	NULL	fatty acid homeostasis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mammalian sirtuin 1 ( SIRT1 ) may control fatty acid homeostasis in liver .
	manualset3
221784	3	420720	7	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Mammalian sirtuin 1 ( SIRT1 ) may control fatty acid homeostasis in liver .
	manualset3
221785	1	420721	7	NULL	NULL	0	NULL	Dative bonding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dative bonding involving O ( 2p ) Th ( 6d ) and U ( df ) interactions is clearly involved in these oxoactinide difluoride molecules .
	manualset3
221786	2	420721	7	NULL	NULL	0	NULL	O ( 2p ) Th ( 6d ) and U ( df ) interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dative bonding involving O ( 2p ) Th ( 6d ) and U ( df ) interactions is clearly involved in these oxoactinide difluoride molecules .
	manualset3
221787	3	420721	7	NULL	NULL	0	NULL	 oxoactinide difluoride molecules	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Dative bonding involving O ( 2p ) Th ( 6d ) and U ( df ) interactions is clearly involved in these oxoactinide difluoride molecules .
	manualset3
221788	1	420722	7	NULL	NULL	NULL	NULL	department of radiology	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To overcome this difficulty , the department of radiology at the University of New Mexico developed a regression-based analysis which ties departmental staffing needs to hospital statistics .
	manualset3
221790	3	420722	7	NULL	NULL	0	NULL	University of New Mexico	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	To overcome this difficulty , the department of radiology at the University of New Mexico developed a regression-based analysis which ties departmental staffing needs to hospital statistics .
	manualset3
221791	4	420722	7	NULL	NULL	0	NULL	regression-based analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To overcome this difficulty , the department of radiology at the University of New Mexico developed a regression-based analysis which ties departmental staffing needs to hospital statistics .
	manualset3
221792	5	420722	7	NULL	NULL	NULL	NULL	departmental staffing needs	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	To overcome this difficulty , the department of radiology at the University of New Mexico developed a regression-based analysis which ties departmental staffing needs to hospital statistics .
	manualset3
221793	6	420722	7	NULL	NULL	0	NULL	hospital statistics	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To overcome this difficulty , the department of radiology at the University of New Mexico developed a regression-based analysis which ties departmental staffing needs to hospital statistics .
	manualset3
226676	7	420722	7	NULL	NULL	0	NULL	difficulty	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To overcome this difficulty , the department of radiology at the University of New Mexico developed a regression-based analysis which ties departmental staffing needs to hospital statistics .
	manualset3
221794	1	420723	7	NULL	NULL	0	NULL	Patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with a large atrial septal defect and tamponade do not manifest a paradoxical pulse .
	manualset3
221795	2	420723	7	NULL	NULL	0	NULL	large atrial septal defect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with a large atrial septal defect and tamponade do not manifest a paradoxical pulse .
	manualset3
221796	3	420723	7	NULL	NULL	0	NULL	tamponade	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with a large atrial septal defect and tamponade do not manifest a paradoxical pulse .
	manualset3
221797	4	420723	7	NULL	NULL	0	NULL	paradoxical pulse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with a large atrial septal defect and tamponade do not manifest a paradoxical pulse .
	manualset3
221798	1	420724	7	NULL	NULL	0	NULL	role 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we examine the role of pilocarpine-induced ERK activation in the induction of seizures in mice by pharmacological and behavioral approaches .
	manualset3
221799	2	420724	7	NULL	NULL	0	NULL	pilocarpine-induced ERK activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we examine the role of pilocarpine-induced ERK activation in the induction of seizures in mice by pharmacological and behavioral approaches .
	manualset3
221800	3	420724	7	NULL	NULL	0	NULL	induction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we examine the role of pilocarpine-induced ERK activation in the induction of seizures in mice by pharmacological and behavioral approaches .
	manualset3
221801	4	420724	7	NULL	NULL	0	NULL	seizures	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we examine the role of pilocarpine-induced ERK activation in the induction of seizures in mice by pharmacological and behavioral approaches .
	manualset3
221802	5	420724	7	NULL	NULL	0	NULL	 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we examine the role of pilocarpine-induced ERK activation in the induction of seizures in mice by pharmacological and behavioral approaches .
	manualset3
221803	6	420724	7	NULL	NULL	0	NULL	pharmacological approaches	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we examine the role of pilocarpine-induced ERK activation in the induction of seizures in mice by pharmacological and behavioral approaches .
	manualset3
221804	7	420724	7	NULL	NULL	0	NULL	behavioral approaches 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we examine the role of pilocarpine-induced ERK activation in the induction of seizures in mice by pharmacological and behavioral approaches .
	manualset3
221805	1	420725	7	NULL	NULL	0	NULL	theory	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Taking the nuances into account , the theory indicates increased usefulness of deplasticized epoxy sections when the diameter of the protein carrying the epitopes decreases .
	manualset3
221806	2	420725	7	NULL	NULL	0	NULL	increased usefulness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Taking the nuances into account , the theory indicates increased usefulness of deplasticized epoxy sections when the diameter of the protein carrying the epitopes decreases .
	manualset3
221807	3	420725	7	NULL	NULL	0	NULL	deplasticized epoxy sections	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Taking the nuances into account , the theory indicates increased usefulness of deplasticized epoxy sections when the diameter of the protein carrying the epitopes decreases .
	manualset3
221808	4	420725	7	NULL	NULL	0	NULL	diameter	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Taking the nuances into account , the theory indicates increased usefulness of deplasticized epoxy sections when the diameter of the protein carrying the epitopes decreases .
	manualset3
221809	5	420725	7	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Taking the nuances into account , the theory indicates increased usefulness of deplasticized epoxy sections when the diameter of the protein carrying the epitopes decreases .
	manualset3
221810	6	420725	7	NULL	NULL	0	NULL	epitopes	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Taking the nuances into account , the theory indicates increased usefulness of deplasticized epoxy sections when the diameter of the protein carrying the epitopes decreases .
	manualset3
223245	7	420725	7	NULL	NULL	0	NULL	account	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Taking the nuances into account , the theory indicates increased usefulness of deplasticized epoxy sections when the diameter of the protein carrying the epitopes decreases .
	manualset3
226677	8	420725	7	NULL	NULL	0	NULL	nuances	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Taking the nuances into account , the theory indicates increased usefulness of deplasticized epoxy sections when the diameter of the protein carrying the epitopes decreases .
	manualset3
221811	1	420726	7	NULL	NULL	0	NULL	Dermatomycosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Dermatomycosis by Microsporum gypseum after unusual infection manner ) .
	manualset3
221812	2	420726	7	NULL	NULL	0	NULL	Microsporum gypseum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Dermatomycosis by Microsporum gypseum after unusual infection manner ) .
	manualset3
221813	3	420726	7	NULL	NULL	0	NULL	unusual infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Dermatomycosis by Microsporum gypseum after unusual infection manner ) .
	manualset3
221814	1	420727	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among children and adolescents , overweight is defined as a body mass index for age at or above the 95th percentile of a specified reference population .
	manualset3
221815	2	420727	7	NULL	NULL	0	NULL	adolescents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among children and adolescents , overweight is defined as a body mass index for age at or above the 95th percentile of a specified reference population .
	manualset3
221816	3	420727	7	NULL	NULL	0	NULL	overweight	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among children and adolescents , overweight is defined as a body mass index for age at or above the 95th percentile of a specified reference population .
	manualset3
221817	4	420727	7	NULL	NULL	0	NULL	body mass index	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among children and adolescents , overweight is defined as a body mass index for age at or above the 95th percentile of a specified reference population .
	manualset3
221818	5	420727	7	NULL	NULL	0	NULL	 age	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among children and adolescents , overweight is defined as a body mass index for age at or above the 95th percentile of a specified reference population .
	manualset3
221819	6	420727	7	NULL	NULL	0	NULL	95th percentile	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among children and adolescents , overweight is defined as a body mass index for age at or above the 95th percentile of a specified reference population .
	manualset3
221820	7	420727	7	NULL	NULL	0	NULL	reference population 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among children and adolescents , overweight is defined as a body mass index for age at or above the 95th percentile of a specified reference population .
	manualset3
221821	1	420728	7	NULL	NULL	0	NULL	One-hundred and forty two individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One-hundred and forty two individuals ( 96 women and 46 men ) , 18-82 yr of age , participated .
	manualset3
221822	2	420728	7	NULL	NULL	0	NULL	96 women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One-hundred and forty two individuals ( 96 women and 46 men ) , 18-82 yr of age , participated .
	manualset3
221823	3	420728	7	NULL	NULL	0	NULL	46 men 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One-hundred and forty two individuals ( 96 women and 46 men ) , 18-82 yr of age , participated .
	manualset3
221824	4	420728	7	NULL	NULL	0	NULL	18-82 yr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	One-hundred and forty two individuals ( 96 women and 46 men ) , 18-82 yr of age , participated .
	manualset3
221825	5	420728	7	NULL	NULL	0	NULL	age	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One-hundred and forty two individuals ( 96 women and 46 men ) , 18-82 yr of age , participated .
	manualset3
221826	1	420729	7	NULL	NULL	0	NULL	 L-5 nerve roots	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The L-5 and L-6 nerve roots were entrapped at the intervertebral foramina between L-5 and the butterfly vertebra ( L-6 ) and between L-6 and S-1 in the concave side .
	manualset3
221827	2	420729	7	NULL	NULL	0	NULL	L-6 nerve roots	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The L-5 and L-6 nerve roots were entrapped at the intervertebral foramina between L-5 and the butterfly vertebra ( L-6 ) and between L-6 and S-1 in the concave side .
	manualset3
221828	3	420729	7	NULL	NULL	0	NULL	intervertebral foramina	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The L-5 and L-6 nerve roots were entrapped at the intervertebral foramina between L-5 and the butterfly vertebra ( L-6 ) and between L-6 and S-1 in the concave side .
	manualset3
221829	4	420729	7	NULL	NULL	0	NULL	L-5	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The L-5 and L-6 nerve roots were entrapped at the intervertebral foramina between L-5 and the butterfly vertebra ( L-6 ) and between L-6 and S-1 in the concave side .
	manualset3
221830	5	420729	7	NULL	NULL	0	NULL	butterfly vertebra ( L-6 )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The L-5 and L-6 nerve roots were entrapped at the intervertebral foramina between L-5 and the butterfly vertebra ( L-6 ) and between L-6 and S-1 in the concave side .
	manualset3
221831	6	420729	7	NULL	NULL	0	NULL	L-6	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The L-5 and L-6 nerve roots were entrapped at the intervertebral foramina between L-5 and the butterfly vertebra ( L-6 ) and between L-6 and S-1 in the concave side .
	manualset3
221832	7	420729	7	NULL	NULL	0	NULL	S-1	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The L-5 and L-6 nerve roots were entrapped at the intervertebral foramina between L-5 and the butterfly vertebra ( L-6 ) and between L-6 and S-1 in the concave side .
	manualset3
221833	8	420729	7	NULL	NULL	0	NULL	concave side	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The L-5 and L-6 nerve roots were entrapped at the intervertebral foramina between L-5 and the butterfly vertebra ( L-6 ) and between L-6 and S-1 in the concave side .
	manualset3
221834	1	420730	7	NULL	NULL	0	NULL	antiplatelet therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Next to antiplatelet therapy , unfractionated heparin ( UFH ) is a well-established concomitant intravenous therapy during PCI .
	manualset3
221835	2	420730	7	NULL	NULL	0	NULL	unfractionated heparin ( UFH )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Next to antiplatelet therapy , unfractionated heparin ( UFH ) is a well-established concomitant intravenous therapy during PCI .
	manualset3
221836	3	420730	7	NULL	NULL	0	NULL	 intravenous therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Next to antiplatelet therapy , unfractionated heparin ( UFH ) is a well-established concomitant intravenous therapy during PCI .
	manualset3
221837	4	420730	7	NULL	NULL	NULL	NULL	PCI	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Next to antiplatelet therapy , unfractionated heparin ( UFH ) is a well-established concomitant intravenous therapy during PCI .
	manualset3
221839	1	420731	7	NULL	NULL	0	NULL	shrink temperature 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The shrink temperature and moisture content of the valvular leaflet and distinct layers of aortic wall of each sample were measured .
	manualset3
221840	2	420731	7	NULL	NULL	0	NULL	moisture content	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The shrink temperature and moisture content of the valvular leaflet and distinct layers of aortic wall of each sample were measured .
	manualset3
221841	3	420731	7	NULL	NULL	0	NULL	valvular leaflet	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The shrink temperature and moisture content of the valvular leaflet and distinct layers of aortic wall of each sample were measured .
	manualset3
221842	4	420731	7	NULL	NULL	0	NULL	distinct layers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The shrink temperature and moisture content of the valvular leaflet and distinct layers of aortic wall of each sample were measured .
	manualset3
221843	5	420731	7	NULL	NULL	0	NULL	aortic wall	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The shrink temperature and moisture content of the valvular leaflet and distinct layers of aortic wall of each sample were measured .
	manualset3
221844	6	420731	7	NULL	NULL	0	NULL	sample	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The shrink temperature and moisture content of the valvular leaflet and distinct layers of aortic wall of each sample were measured .
	manualset3
221845	1	420732	7	NULL	NULL	0	NULL	case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of acute posterior multifocal placoid pigment epitheliopathy is presented with the unusual feature of the exposure of deep choroidal vessels which filled with dye in the early phase of the fluorescein angiogram in the center of many of the placoid lesions .
	manualset3
221846	2	420732	7	NULL	NULL	0	NULL	posterior multifocal placoid pigment epitheliopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of acute posterior multifocal placoid pigment epitheliopathy is presented with the unusual feature of the exposure of deep choroidal vessels which filled with dye in the early phase of the fluorescein angiogram in the center of many of the placoid lesions .
	manualset3
221847	3	420732	7	NULL	NULL	0	NULL	unusual feature 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of acute posterior multifocal placoid pigment epitheliopathy is presented with the unusual feature of the exposure of deep choroidal vessels which filled with dye in the early phase of the fluorescein angiogram in the center of many of the placoid lesions .
	manualset3
221848	4	420732	7	NULL	NULL	0	NULL	exposure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of acute posterior multifocal placoid pigment epitheliopathy is presented with the unusual feature of the exposure of deep choroidal vessels which filled with dye in the early phase of the fluorescein angiogram in the center of many of the placoid lesions .
	manualset3
221850	5	420732	7	NULL	NULL	0	NULL	deep choroidal vessels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of acute posterior multifocal placoid pigment epitheliopathy is presented with the unusual feature of the exposure of deep choroidal vessels which filled with dye in the early phase of the fluorescein angiogram in the center of many of the placoid lesions .
	manualset3
221851	6	420732	7	NULL	NULL	0	NULL	dye	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of acute posterior multifocal placoid pigment epitheliopathy is presented with the unusual feature of the exposure of deep choroidal vessels which filled with dye in the early phase of the fluorescein angiogram in the center of many of the placoid lesions .
	manualset3
221852	7	420732	7	NULL	NULL	0	NULL	early phase	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of acute posterior multifocal placoid pigment epitheliopathy is presented with the unusual feature of the exposure of deep choroidal vessels which filled with dye in the early phase of the fluorescein angiogram in the center of many of the placoid lesions .
	manualset3
221853	8	420732	7	NULL	NULL	0	NULL	fluorescein angiogram	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of acute posterior multifocal placoid pigment epitheliopathy is presented with the unusual feature of the exposure of deep choroidal vessels which filled with dye in the early phase of the fluorescein angiogram in the center of many of the placoid lesions .
	manualset3
221854	9	420732	7	NULL	NULL	0	NULL	center	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of acute posterior multifocal placoid pigment epitheliopathy is presented with the unusual feature of the exposure of deep choroidal vessels which filled with dye in the early phase of the fluorescein angiogram in the center of many of the placoid lesions .
	manualset3
221855	10	420732	7	NULL	NULL	0	NULL	placoid lesions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A case of acute posterior multifocal placoid pigment epitheliopathy is presented with the unusual feature of the exposure of deep choroidal vessels which filled with dye in the early phase of the fluorescein angiogram in the center of many of the placoid lesions .
	manualset3
221856	1	420733	7	NULL	NULL	0	NULL	Schober tests	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Both Schober tests and measurements of lumbar and cervical rotations ( TRi , TR , CR , CRt ) and lateral flexions ( LFLf , LFLx , CLFLt , CLFLm ) , together with thoracolumbar flexion ( ThFL ) , cervical flexion-extension measurements ( CFL , CExt ) , and tragus - wall and occiput - wall distances ( OWD , TWD ) , showed significant correlations with detailed radiological spinal changes .
	manualset3
221857	2	420733	7	NULL	NULL	0	NULL	measurements	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Both Schober tests and measurements of lumbar and cervical rotations ( TRi , TR , CR , CRt ) and lateral flexions ( LFLf , LFLx , CLFLt , CLFLm ) , together with thoracolumbar flexion ( ThFL ) , cervical flexion-extension measurements ( CFL , CExt ) , and tragus - wall and occiput - wall distances ( OWD , TWD ) , showed significant correlations with detailed radiological spinal changes .
	manualset3
221859	3	420733	7	NULL	NULL	0	NULL	lumbar rotations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Both Schober tests and measurements of lumbar and cervical rotations ( TRi , TR , CR , CRt ) and lateral flexions ( LFLf , LFLx , CLFLt , CLFLm ) , together with thoracolumbar flexion ( ThFL ) , cervical flexion-extension measurements ( CFL , CExt ) , and tragus - wall and occiput - wall distances ( OWD , TWD ) , showed significant correlations with detailed radiological spinal changes .
	manualset3
221860	4	420733	7	NULL	NULL	0	NULL	cervical rotations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Both Schober tests and measurements of lumbar and cervical rotations ( TRi , TR , CR , CRt ) and lateral flexions ( LFLf , LFLx , CLFLt , CLFLm ) , together with thoracolumbar flexion ( ThFL ) , cervical flexion-extension measurements ( CFL , CExt ) , and tragus - wall and occiput - wall distances ( OWD , TWD ) , showed significant correlations with detailed radiological spinal changes .
	manualset3
221863	5	420733	7	NULL	NULL	0	NULL	TRi	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Both Schober tests and measurements of lumbar and cervical rotations ( TRi , TR , CR , CRt ) and lateral flexions ( LFLf , LFLx , CLFLt , CLFLm ) , together with thoracolumbar flexion ( ThFL ) , cervical flexion-extension measurements ( CFL , CExt ) , and tragus - wall and occiput - wall distances ( OWD , TWD ) , showed significant correlations with detailed radiological spinal changes .
	manualset3
221864	6	420733	7	NULL	NULL	0	NULL	TR	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Both Schober tests and measurements of lumbar and cervical rotations ( TRi , TR , CR , CRt ) and lateral flexions ( LFLf , LFLx , CLFLt , CLFLm ) , together with thoracolumbar flexion ( ThFL ) , cervical flexion-extension measurements ( CFL , CExt ) , and tragus - wall and occiput - wall distances ( OWD , TWD ) , showed significant correlations with detailed radiological spinal changes .
	manualset3
221865	7	420733	7	NULL	NULL	0	NULL	CR	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Both Schober tests and measurements of lumbar and cervical rotations ( TRi , TR , CR , CRt ) and lateral flexions ( LFLf , LFLx , CLFLt , CLFLm ) , together with thoracolumbar flexion ( ThFL ) , cervical flexion-extension measurements ( CFL , CExt ) , and tragus - wall and occiput - wall distances ( OWD , TWD ) , showed significant correlations with detailed radiological spinal changes .
	manualset3
221866	8	420733	7	NULL	NULL	0	NULL	CRt	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Both Schober tests and measurements of lumbar and cervical rotations ( TRi , TR , CR , CRt ) and lateral flexions ( LFLf , LFLx , CLFLt , CLFLm ) , together with thoracolumbar flexion ( ThFL ) , cervical flexion-extension measurements ( CFL , CExt ) , and tragus - wall and occiput - wall distances ( OWD , TWD ) , showed significant correlations with detailed radiological spinal changes .
	manualset3
221867	9	420733	7	NULL	NULL	0	NULL	lateral flexions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Both Schober tests and measurements of lumbar and cervical rotations ( TRi , TR , CR , CRt ) and lateral flexions ( LFLf , LFLx , CLFLt , CLFLm ) , together with thoracolumbar flexion ( ThFL ) , cervical flexion-extension measurements ( CFL , CExt ) , and tragus - wall and occiput - wall distances ( OWD , TWD ) , showed significant correlations with detailed radiological spinal changes .
	manualset3
221868	10	420733	7	NULL	NULL	0	NULL	LFLf	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Both Schober tests and measurements of lumbar and cervical rotations ( TRi , TR , CR , CRt ) and lateral flexions ( LFLf , LFLx , CLFLt , CLFLm ) , together with thoracolumbar flexion ( ThFL ) , cervical flexion-extension measurements ( CFL , CExt ) , and tragus - wall and occiput - wall distances ( OWD , TWD ) , showed significant correlations with detailed radiological spinal changes .
	manualset3
221869	11	420733	7	NULL	NULL	0	NULL	LFLx	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Both Schober tests and measurements of lumbar and cervical rotations ( TRi , TR , CR , CRt ) and lateral flexions ( LFLf , LFLx , CLFLt , CLFLm ) , together with thoracolumbar flexion ( ThFL ) , cervical flexion-extension measurements ( CFL , CExt ) , and tragus - wall and occiput - wall distances ( OWD , TWD ) , showed significant correlations with detailed radiological spinal changes .
	manualset3
221870	12	420733	7	NULL	NULL	0	NULL	CLFLt	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Both Schober tests and measurements of lumbar and cervical rotations ( TRi , TR , CR , CRt ) and lateral flexions ( LFLf , LFLx , CLFLt , CLFLm ) , together with thoracolumbar flexion ( ThFL ) , cervical flexion-extension measurements ( CFL , CExt ) , and tragus - wall and occiput - wall distances ( OWD , TWD ) , showed significant correlations with detailed radiological spinal changes .
	manualset3
221871	13	420733	7	NULL	NULL	0	NULL	CLFLm	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Both Schober tests and measurements of lumbar and cervical rotations ( TRi , TR , CR , CRt ) and lateral flexions ( LFLf , LFLx , CLFLt , CLFLm ) , together with thoracolumbar flexion ( ThFL ) , cervical flexion-extension measurements ( CFL , CExt ) , and tragus - wall and occiput - wall distances ( OWD , TWD ) , showed significant correlations with detailed radiological spinal changes .
	manualset3
221872	14	420733	7	NULL	NULL	NULL	NULL	thoracolumbar flexion 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Both Schober tests and measurements of lumbar and cervical rotations ( TRi , TR , CR , CRt ) and lateral flexions ( LFLf , LFLx , CLFLt , CLFLm ) , together with thoracolumbar flexion ( ThFL ) , cervical flexion-extension measurements ( CFL , CExt ) , and tragus - wall and occiput - wall distances ( OWD , TWD ) , showed significant correlations with detailed radiological spinal changes .
	manualset3
221873	15	420733	7	NULL	NULL	0	NULL	ThFL	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Both Schober tests and measurements of lumbar and cervical rotations ( TRi , TR , CR , CRt ) and lateral flexions ( LFLf , LFLx , CLFLt , CLFLm ) , together with thoracolumbar flexion ( ThFL ) , cervical flexion-extension measurements ( CFL , CExt ) , and tragus - wall and occiput - wall distances ( OWD , TWD ) , showed significant correlations with detailed radiological spinal changes .
	manualset3
221874	16	420733	7	NULL	NULL	0	NULL	cervical flexion-extension measurements 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Both Schober tests and measurements of lumbar and cervical rotations ( TRi , TR , CR , CRt ) and lateral flexions ( LFLf , LFLx , CLFLt , CLFLm ) , together with thoracolumbar flexion ( ThFL ) , cervical flexion-extension measurements ( CFL , CExt ) , and tragus - wall and occiput - wall distances ( OWD , TWD ) , showed significant correlations with detailed radiological spinal changes .
	manualset3
221875	17	420733	7	NULL	NULL	0	NULL	CFL	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Both Schober tests and measurements of lumbar and cervical rotations ( TRi , TR , CR , CRt ) and lateral flexions ( LFLf , LFLx , CLFLt , CLFLm ) , together with thoracolumbar flexion ( ThFL ) , cervical flexion-extension measurements ( CFL , CExt ) , and tragus - wall and occiput - wall distances ( OWD , TWD ) , showed significant correlations with detailed radiological spinal changes .
	manualset3
221876	18	420733	7	NULL	NULL	0	NULL	CExt 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Both Schober tests and measurements of lumbar and cervical rotations ( TRi , TR , CR , CRt ) and lateral flexions ( LFLf , LFLx , CLFLt , CLFLm ) , together with thoracolumbar flexion ( ThFL ) , cervical flexion-extension measurements ( CFL , CExt ) , and tragus - wall and occiput - wall distances ( OWD , TWD ) , showed significant correlations with detailed radiological spinal changes .
	manualset3
221877	19	420733	7	NULL	NULL	0	NULL	tragus - wall distances	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Both Schober tests and measurements of lumbar and cervical rotations ( TRi , TR , CR , CRt ) and lateral flexions ( LFLf , LFLx , CLFLt , CLFLm ) , together with thoracolumbar flexion ( ThFL ) , cervical flexion-extension measurements ( CFL , CExt ) , and tragus - wall and occiput - wall distances ( OWD , TWD ) , showed significant correlations with detailed radiological spinal changes .
	manualset3
221878	20	420733	7	NULL	NULL	0	NULL	occiput - wall distances	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Both Schober tests and measurements of lumbar and cervical rotations ( TRi , TR , CR , CRt ) and lateral flexions ( LFLf , LFLx , CLFLt , CLFLm ) , together with thoracolumbar flexion ( ThFL ) , cervical flexion-extension measurements ( CFL , CExt ) , and tragus - wall and occiput - wall distances ( OWD , TWD ) , showed significant correlations with detailed radiological spinal changes .
	manualset3
221879	21	420733	7	NULL	NULL	0	NULL	OWD	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Both Schober tests and measurements of lumbar and cervical rotations ( TRi , TR , CR , CRt ) and lateral flexions ( LFLf , LFLx , CLFLt , CLFLm ) , together with thoracolumbar flexion ( ThFL ) , cervical flexion-extension measurements ( CFL , CExt ) , and tragus - wall and occiput - wall distances ( OWD , TWD ) , showed significant correlations with detailed radiological spinal changes .
	manualset3
221880	22	420733	7	NULL	NULL	0	NULL	TWD	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Both Schober tests and measurements of lumbar and cervical rotations ( TRi , TR , CR , CRt ) and lateral flexions ( LFLf , LFLx , CLFLt , CLFLm ) , together with thoracolumbar flexion ( ThFL ) , cervical flexion-extension measurements ( CFL , CExt ) , and tragus - wall and occiput - wall distances ( OWD , TWD ) , showed significant correlations with detailed radiological spinal changes .
	manualset3
221881	23	420733	7	NULL	NULL	0	NULL	correlations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Both Schober tests and measurements of lumbar and cervical rotations ( TRi , TR , CR , CRt ) and lateral flexions ( LFLf , LFLx , CLFLt , CLFLm ) , together with thoracolumbar flexion ( ThFL ) , cervical flexion-extension measurements ( CFL , CExt ) , and tragus - wall and occiput - wall distances ( OWD , TWD ) , showed significant correlations with detailed radiological spinal changes .
	manualset3
221882	24	420733	7	NULL	NULL	0	NULL	radiological spinal changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Both Schober tests and measurements of lumbar and cervical rotations ( TRi , TR , CR , CRt ) and lateral flexions ( LFLf , LFLx , CLFLt , CLFLm ) , together with thoracolumbar flexion ( ThFL ) , cervical flexion-extension measurements ( CFL , CExt ) , and tragus - wall and occiput - wall distances ( OWD , TWD ) , showed significant correlations with detailed radiological spinal changes .
	manualset3
221883	1	420734	7	NULL	NULL	0	NULL	 nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The nucleus showed increasing condensation of chromatin at the periphery and clearing of the center .
	manualset3
221884	2	420734	7	NULL	NULL	0	NULL	 increasing condensation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The nucleus showed increasing condensation of chromatin at the periphery and clearing of the center .
	manualset3
221885	3	420734	7	NULL	NULL	0	NULL	chromatin	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The nucleus showed increasing condensation of chromatin at the periphery and clearing of the center .
	manualset3
221886	4	420734	7	NULL	NULL	0	NULL	periphery	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The nucleus showed increasing condensation of chromatin at the periphery and clearing of the center .
	manualset3
221887	5	420734	7	NULL	NULL	0	NULL	clearing of the center	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	The nucleus showed increasing condensation of chromatin at the periphery and clearing of the center .
	manualset3
221888	1	420735	7	NULL	NULL	0	NULL	 investigations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Further investigations are needed to delineate the clinical spectrum of features essential for partial trisomy 4q .
	manualset3
221889	2	420735	7	NULL	NULL	0	NULL	clinical spectrum	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Further investigations are needed to delineate the clinical spectrum of features essential for partial trisomy 4q .
	manualset3
221890	3	420735	7	NULL	NULL	0	NULL	features	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Further investigations are needed to delineate the clinical spectrum of features essential for partial trisomy 4q .
	manualset3
221891	4	420735	7	NULL	NULL	0	NULL	partial trisomy 4q	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Further investigations are needed to delineate the clinical spectrum of features essential for partial trisomy 4q .
	manualset3
221892	1	420736	7	NULL	NULL	0	NULL	association 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The association of hepatic glycogen depletion with hyperammonemia in cirrhosis .
	manualset3
221893	2	420736	7	NULL	NULL	0	NULL	hepatic glycogen depletion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The association of hepatic glycogen depletion with hyperammonemia in cirrhosis .
	manualset3
221894	3	420736	7	NULL	NULL	0	NULL	hyperammonemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The association of hepatic glycogen depletion with hyperammonemia in cirrhosis .
	manualset3
221895	4	420736	7	NULL	NULL	0	NULL	cirrhosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The association of hepatic glycogen depletion with hyperammonemia in cirrhosis .
	manualset3
221896	1	420737	7	NULL	NULL	0	NULL	college women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among college women , positive experiences with mother also were linked to better relationship functioning ; however , attachment style and depression status mediated this effect .
	manualset3
221897	2	420737	7	NULL	NULL	0	NULL	positive experiences	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among college women , positive experiences with mother also were linked to better relationship functioning ; however , attachment style and depression status mediated this effect .
	manualset3
221898	3	420737	7	NULL	NULL	0	NULL	mother	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Among college women , positive experiences with mother also were linked to better relationship functioning ; however , attachment style and depression status mediated this effect .
	manualset3
221899	4	420737	7	NULL	NULL	0	NULL	attachment style 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among college women , positive experiences with mother also were linked to better relationship functioning ; however , attachment style and depression status mediated this effect .
	manualset3
221900	5	420737	7	NULL	NULL	0	NULL	depression status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among college women , positive experiences with mother also were linked to better relationship functioning ; however , attachment style and depression status mediated this effect .
	manualset3
221901	6	420737	7	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among college women , positive experiences with mother also were linked to better relationship functioning ; however , attachment style and depression status mediated this effect .
	manualset3
221902	7	420737	7	NULL	NULL	0	NULL	 relationship functioning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among college women , positive experiences with mother also were linked to better relationship functioning ; however , attachment style and depression status mediated this effect .
	manualset3
221903	1	420738	7	NULL	NULL	0	NULL	 example	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , point mutations often lead to substantial flexibility increases within the - subdomain , which is consistent with experimental results indicating that it is the nucleation site for amyloid formation .
	manualset3
221904	2	420738	7	NULL	NULL	0	NULL	point mutations 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , point mutations often lead to substantial flexibility increases within the - subdomain , which is consistent with experimental results indicating that it is the nucleation site for amyloid formation .
	manualset3
221905	3	420738	7	NULL	NULL	0	NULL	substantial flexibility 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , point mutations often lead to substantial flexibility increases within the - subdomain , which is consistent with experimental results indicating that it is the nucleation site for amyloid formation .
	manualset3
221906	4	420738	7	NULL	NULL	0	NULL	subdomain 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , point mutations often lead to substantial flexibility increases within the - subdomain , which is consistent with experimental results indicating that it is the nucleation site for amyloid formation .
	manualset3
221907	5	420738	7	NULL	NULL	0	NULL	experimental results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , point mutations often lead to substantial flexibility increases within the - subdomain , which is consistent with experimental results indicating that it is the nucleation site for amyloid formation .
	manualset3
221908	6	420738	7	NULL	NULL	0	NULL	 nucleation site 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , point mutations often lead to substantial flexibility increases within the - subdomain , which is consistent with experimental results indicating that it is the nucleation site for amyloid formation .
	manualset3
221909	7	420738	7	NULL	NULL	0	NULL	amyloid formation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , point mutations often lead to substantial flexibility increases within the - subdomain , which is consistent with experimental results indicating that it is the nucleation site for amyloid formation .
	manualset3
221910	1	420739	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effects of success and failure on control effort ) .
	manualset3
221911	2	420739	7	NULL	NULL	0	NULL	success	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effects of success and failure on control effort ) .
	manualset3
221912	3	420739	7	NULL	NULL	0	NULL	failure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effects of success and failure on control effort ) .
	manualset3
221913	4	420739	7	NULL	NULL	0	NULL	control effort	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effects of success and failure on control effort ) .
	manualset3
221914	1	420740	7	NULL	NULL	0	NULL	Mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the purine nucleotide binding ( PNB ) site weakened each of the protein 's abilities to repress expression .
	manualset3
221915	2	420740	7	NULL	NULL	0	NULL	purine nucleotide binding ( PNB ) site 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the purine nucleotide binding ( PNB ) site weakened each of the protein 's abilities to repress expression .
	manualset3
221916	3	420740	7	NULL	NULL	0	NULL	protein 's abilities 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the purine nucleotide binding ( PNB ) site weakened each of the protein 's abilities to repress expression .
	manualset3
221917	4	420740	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in the purine nucleotide binding ( PNB ) site weakened each of the protein 's abilities to repress expression .
	manualset3
221918	1	420741	7	NULL	NULL	0	NULL	Genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Genes coding for RNA-polymerase in bacteria .
	manualset3
221919	2	420741	7	NULL	NULL	0	NULL	RNA-polymerase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Genes coding for RNA-polymerase in bacteria .
	manualset3
221920	3	420741	7	NULL	NULL	0	NULL	bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Genes coding for RNA-polymerase in bacteria .
	manualset3
221921	1	420742	7	NULL	NULL	0	NULL	Detection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Detection of pairwise residue proximity by covariation analysis for 3D-structure prediction of G-protein-coupled receptors .
	manualset3
221922	2	420742	7	NULL	NULL	0	NULL	pairwise residue proximity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Detection of pairwise residue proximity by covariation analysis for 3D-structure prediction of G-protein-coupled receptors .
	manualset3
221923	3	420742	7	NULL	NULL	0	NULL	covariation analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Detection of pairwise residue proximity by covariation analysis for 3D-structure prediction of G-protein-coupled receptors .
	manualset3
221924	4	420742	7	NULL	NULL	0	NULL	3D-structure prediction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Detection of pairwise residue proximity by covariation analysis for 3D-structure prediction of G-protein-coupled receptors .
	manualset3
221925	5	420742	7	NULL	NULL	0	NULL	G-protein-coupled receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Detection of pairwise residue proximity by covariation analysis for 3D-structure prediction of G-protein-coupled receptors .
	manualset3
221926	1	420743	7	NULL	NULL	0	NULL	Vascular lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Vascular lesions resembling polyarteritis nodosa in rats undergoing prolonged stimulation with estrogen .
	manualset3
221927	2	420743	7	NULL	NULL	0	NULL	polyarteritis nodosa	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Vascular lesions resembling polyarteritis nodosa in rats undergoing prolonged stimulation with estrogen .
	manualset3
221928	3	420743	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Vascular lesions resembling polyarteritis nodosa in rats undergoing prolonged stimulation with estrogen .
	manualset3
221929	4	420743	7	NULL	NULL	0	NULL	prolonged stimulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Vascular lesions resembling polyarteritis nodosa in rats undergoing prolonged stimulation with estrogen .
	manualset3
221930	5	420743	7	NULL	NULL	0	NULL	estrogen	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Vascular lesions resembling polyarteritis nodosa in rats undergoing prolonged stimulation with estrogen .
	manualset3
221931	1	420744	7	NULL	NULL	NULL	NULL	intermittent incremental protocols	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was concluded that it is valid to use intermittent incremental protocols of 200 and 300 m lengths to assess the swimming velocity corresponding to individual anaerobic threshold , the progressive protocols tend to underestimate the ( La - ) at anaerobic threshold assessed by the MLSS test , and swimmers increase velocity through stroke rate increases .
	manualset3
221932	2	420744	7	NULL	NULL	0	NULL	200 m lengths	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that it is valid to use intermittent incremental protocols of 200 and 300 m lengths to assess the swimming velocity corresponding to individual anaerobic threshold , the progressive protocols tend to underestimate the ( La - ) at anaerobic threshold assessed by the MLSS test , and swimmers increase velocity through stroke rate increases .
	manualset3
221933	3	420744	7	NULL	NULL	0	NULL	 300 m lengths	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that it is valid to use intermittent incremental protocols of 200 and 300 m lengths to assess the swimming velocity corresponding to individual anaerobic threshold , the progressive protocols tend to underestimate the ( La - ) at anaerobic threshold assessed by the MLSS test , and swimmers increase velocity through stroke rate increases .
	manualset3
221934	4	420744	7	NULL	NULL	0	NULL	swimming velocity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that it is valid to use intermittent incremental protocols of 200 and 300 m lengths to assess the swimming velocity corresponding to individual anaerobic threshold , the progressive protocols tend to underestimate the ( La - ) at anaerobic threshold assessed by the MLSS test , and swimmers increase velocity through stroke rate increases .
	manualset3
221935	5	420744	7	NULL	NULL	0	NULL	individual anaerobic threshold 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that it is valid to use intermittent incremental protocols of 200 and 300 m lengths to assess the swimming velocity corresponding to individual anaerobic threshold , the progressive protocols tend to underestimate the ( La - ) at anaerobic threshold assessed by the MLSS test , and swimmers increase velocity through stroke rate increases .
	manualset3
221936	6	420744	7	NULL	NULL	NULL	NULL	progressive protocols	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was concluded that it is valid to use intermittent incremental protocols of 200 and 300 m lengths to assess the swimming velocity corresponding to individual anaerobic threshold , the progressive protocols tend to underestimate the ( La - ) at anaerobic threshold assessed by the MLSS test , and swimmers increase velocity through stroke rate increases .
	manualset3
221937	7	420744	7	NULL	NULL	0	NULL	La - 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that it is valid to use intermittent incremental protocols of 200 and 300 m lengths to assess the swimming velocity corresponding to individual anaerobic threshold , the progressive protocols tend to underestimate the ( La - ) at anaerobic threshold assessed by the MLSS test , and swimmers increase velocity through stroke rate increases .
	manualset3
221938	8	420744	7	NULL	NULL	0	NULL	anaerobic threshold 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that it is valid to use intermittent incremental protocols of 200 and 300 m lengths to assess the swimming velocity corresponding to individual anaerobic threshold , the progressive protocols tend to underestimate the ( La - ) at anaerobic threshold assessed by the MLSS test , and swimmers increase velocity through stroke rate increases .
	manualset3
221939	9	420744	7	NULL	NULL	NULL	NULL	MLSS test	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It was concluded that it is valid to use intermittent incremental protocols of 200 and 300 m lengths to assess the swimming velocity corresponding to individual anaerobic threshold , the progressive protocols tend to underestimate the ( La - ) at anaerobic threshold assessed by the MLSS test , and swimmers increase velocity through stroke rate increases .
	manualset3
221940	10	420744	7	NULL	NULL	0	NULL	swimmers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that it is valid to use intermittent incremental protocols of 200 and 300 m lengths to assess the swimming velocity corresponding to individual anaerobic threshold , the progressive protocols tend to underestimate the ( La - ) at anaerobic threshold assessed by the MLSS test , and swimmers increase velocity through stroke rate increases .
	manualset3
221941	11	420744	7	NULL	NULL	0	NULL	velocity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that it is valid to use intermittent incremental protocols of 200 and 300 m lengths to assess the swimming velocity corresponding to individual anaerobic threshold , the progressive protocols tend to underestimate the ( La - ) at anaerobic threshold assessed by the MLSS test , and swimmers increase velocity through stroke rate increases .
	manualset3
221942	12	420744	7	NULL	NULL	0	NULL	stroke rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It was concluded that it is valid to use intermittent incremental protocols of 200 and 300 m lengths to assess the swimming velocity corresponding to individual anaerobic threshold , the progressive protocols tend to underestimate the ( La - ) at anaerobic threshold assessed by the MLSS test , and swimmers increase velocity through stroke rate increases .
	manualset3
221943	1	420745	7	NULL	NULL	0	NULL	Fluorescence induction and relaxation ( FIRe ) fluorometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescence induction and relaxation ( FIRe ) fluorometry and Fourier transform infrared spectroscopy ( FTIR ) were used to monitor the photosynthetic performance , lipid production and metabolic responses to changing N availability .
	manualset3
221944	2	420745	7	NULL	NULL	0	NULL	Fourier transform infrared spectroscopy ( FTIR )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescence induction and relaxation ( FIRe ) fluorometry and Fourier transform infrared spectroscopy ( FTIR ) were used to monitor the photosynthetic performance , lipid production and metabolic responses to changing N availability .
	manualset3
221946	3	420745	7	NULL	NULL	0	NULL	photosynthetic performance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescence induction and relaxation ( FIRe ) fluorometry and Fourier transform infrared spectroscopy ( FTIR ) were used to monitor the photosynthetic performance , lipid production and metabolic responses to changing N availability .
	manualset3
221947	4	420745	7	NULL	NULL	0	NULL	lipid production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescence induction and relaxation ( FIRe ) fluorometry and Fourier transform infrared spectroscopy ( FTIR ) were used to monitor the photosynthetic performance , lipid production and metabolic responses to changing N availability .
	manualset3
221948	5	420745	7	NULL	NULL	0	NULL	metabolic responses	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescence induction and relaxation ( FIRe ) fluorometry and Fourier transform infrared spectroscopy ( FTIR ) were used to monitor the photosynthetic performance , lipid production and metabolic responses to changing N availability .
	manualset3
221950	6	420745	7	NULL	NULL	0	NULL	N availability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescence induction and relaxation ( FIRe ) fluorometry and Fourier transform infrared spectroscopy ( FTIR ) were used to monitor the photosynthetic performance , lipid production and metabolic responses to changing N availability .
	manualset3
221958	1	420746	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When mice treated intracerebrally with adenoviruses expressing siRNAs were challenged peripherally with lethal RABV by the intramuscular route in masseter muscle , there was 66.6 % and 33.3 % protection with adenoviruses expressing siRNAs against RABV-N and L genes , respectively .
	manualset3
221959	2	420746	7	NULL	NULL	0	NULL	adenoviruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When mice treated intracerebrally with adenoviruses expressing siRNAs were challenged peripherally with lethal RABV by the intramuscular route in masseter muscle , there was 66.6 % and 33.3 % protection with adenoviruses expressing siRNAs against RABV-N and L genes , respectively .
	manualset3
221960	3	420746	7	NULL	NULL	0	NULL	siRNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	When mice treated intracerebrally with adenoviruses expressing siRNAs were challenged peripherally with lethal RABV by the intramuscular route in masseter muscle , there was 66.6 % and 33.3 % protection with adenoviruses expressing siRNAs against RABV-N and L genes , respectively .
	manualset3
221961	4	420746	7	NULL	NULL	0	NULL	lethal RABV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When mice treated intracerebrally with adenoviruses expressing siRNAs were challenged peripherally with lethal RABV by the intramuscular route in masseter muscle , there was 66.6 % and 33.3 % protection with adenoviruses expressing siRNAs against RABV-N and L genes , respectively .
	manualset3
221962	5	420746	7	NULL	NULL	0	NULL	 intramuscular route	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	When mice treated intracerebrally with adenoviruses expressing siRNAs were challenged peripherally with lethal RABV by the intramuscular route in masseter muscle , there was 66.6 % and 33.3 % protection with adenoviruses expressing siRNAs against RABV-N and L genes , respectively .
	manualset3
221963	6	420746	7	NULL	NULL	0	NULL	masseter muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When mice treated intracerebrally with adenoviruses expressing siRNAs were challenged peripherally with lethal RABV by the intramuscular route in masseter muscle , there was 66.6 % and 33.3 % protection with adenoviruses expressing siRNAs against RABV-N and L genes , respectively .
	manualset3
221964	7	420746	7	NULL	NULL	0	NULL	66.6 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When mice treated intracerebrally with adenoviruses expressing siRNAs were challenged peripherally with lethal RABV by the intramuscular route in masseter muscle , there was 66.6 % and 33.3 % protection with adenoviruses expressing siRNAs against RABV-N and L genes , respectively .
	manualset3
221965	8	420746	7	NULL	NULL	0	NULL	33.3 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When mice treated intracerebrally with adenoviruses expressing siRNAs were challenged peripherally with lethal RABV by the intramuscular route in masseter muscle , there was 66.6 % and 33.3 % protection with adenoviruses expressing siRNAs against RABV-N and L genes , respectively .
	manualset3
221966	9	420746	7	NULL	NULL	0	NULL	protection 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When mice treated intracerebrally with adenoviruses expressing siRNAs were challenged peripherally with lethal RABV by the intramuscular route in masseter muscle , there was 66.6 % and 33.3 % protection with adenoviruses expressing siRNAs against RABV-N and L genes , respectively .
	manualset3
221967	10	420746	7	NULL	NULL	0	NULL	adenoviruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When mice treated intracerebrally with adenoviruses expressing siRNAs were challenged peripherally with lethal RABV by the intramuscular route in masseter muscle , there was 66.6 % and 33.3 % protection with adenoviruses expressing siRNAs against RABV-N and L genes , respectively .
	manualset3
221968	11	420746	7	NULL	NULL	0	NULL	siRNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	When mice treated intracerebrally with adenoviruses expressing siRNAs were challenged peripherally with lethal RABV by the intramuscular route in masseter muscle , there was 66.6 % and 33.3 % protection with adenoviruses expressing siRNAs against RABV-N and L genes , respectively .
	manualset3
221969	12	420746	7	NULL	NULL	0	NULL	RABV-N genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When mice treated intracerebrally with adenoviruses expressing siRNAs were challenged peripherally with lethal RABV by the intramuscular route in masseter muscle , there was 66.6 % and 33.3 % protection with adenoviruses expressing siRNAs against RABV-N and L genes , respectively .
	manualset3
221970	13	420746	7	NULL	NULL	0	NULL	L genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When mice treated intracerebrally with adenoviruses expressing siRNAs were challenged peripherally with lethal RABV by the intramuscular route in masseter muscle , there was 66.6 % and 33.3 % protection with adenoviruses expressing siRNAs against RABV-N and L genes , respectively .
	manualset3
221971	1	420747	7	NULL	NULL	0	NULL	Preventive measures 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Preventive measures , which reduced the salivary level of mutans streptococci in mothers , delayed colonization by these organisms in their children .
	manualset3
221972	2	420747	7	NULL	NULL	0	NULL	salivary level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Preventive measures , which reduced the salivary level of mutans streptococci in mothers , delayed colonization by these organisms in their children .
	manualset3
221973	3	420747	7	NULL	NULL	0	NULL	mutans streptococci	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Preventive measures , which reduced the salivary level of mutans streptococci in mothers , delayed colonization by these organisms in their children .
	manualset3
221974	4	420747	7	NULL	NULL	0	NULL	mothers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Preventive measures , which reduced the salivary level of mutans streptococci in mothers , delayed colonization by these organisms in their children .
	manualset3
221975	5	420747	7	NULL	NULL	NULL	NULL	colonization	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Preventive measures , which reduced the salivary level of mutans streptococci in mothers , delayed colonization by these organisms in their children .
	manualset3
221976	6	420747	7	NULL	NULL	0	NULL	organisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Preventive measures , which reduced the salivary level of mutans streptococci in mothers , delayed colonization by these organisms in their children .
	manualset3
221977	7	420747	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Preventive measures , which reduced the salivary level of mutans streptococci in mothers , delayed colonization by these organisms in their children .
	manualset3
221978	1	420748	7	NULL	NULL	0	NULL	Transgenic mouse blastocysts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Transgenic mouse blastocysts that overexpress metallothionein-I resist cadmium toxicity in vitro .
	manualset3
221979	2	420748	7	NULL	NULL	0	NULL	 metallothionein-I resist cadmium toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Transgenic mouse blastocysts that overexpress metallothionein-I resist cadmium toxicity in vitro .
	manualset3
221980	1	420749	7	NULL	NULL	0	NULL	Alpha-adrenergic blockade	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Alpha-adrenergic blockade with dibenzyline prevented the GSR produced by endotoxin in rats , whether pregnant , diabetic , or having a unilateral ureteral occlusion , and the classic reaction in rabbits , but not that produced in renal-hypertensive rats .
	manualset3
221981	2	420749	7	NULL	NULL	0	NULL	dibenzyline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Alpha-adrenergic blockade with dibenzyline prevented the GSR produced by endotoxin in rats , whether pregnant , diabetic , or having a unilateral ureteral occlusion , and the classic reaction in rabbits , but not that produced in renal-hypertensive rats .
	manualset3
221982	3	420749	7	NULL	NULL	0	NULL	 GSR	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Alpha-adrenergic blockade with dibenzyline prevented the GSR produced by endotoxin in rats , whether pregnant , diabetic , or having a unilateral ureteral occlusion , and the classic reaction in rabbits , but not that produced in renal-hypertensive rats .
	manualset3
221983	4	420749	7	NULL	NULL	0	NULL	endotoxin	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Alpha-adrenergic blockade with dibenzyline prevented the GSR produced by endotoxin in rats , whether pregnant , diabetic , or having a unilateral ureteral occlusion , and the classic reaction in rabbits , but not that produced in renal-hypertensive rats .
	manualset3
221984	5	420749	7	NULL	NULL	0	NULL	 rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Alpha-adrenergic blockade with dibenzyline prevented the GSR produced by endotoxin in rats , whether pregnant , diabetic , or having a unilateral ureteral occlusion , and the classic reaction in rabbits , but not that produced in renal-hypertensive rats .
	manualset3
221985	6	420749	7	NULL	NULL	0	NULL	pregnant 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Alpha-adrenergic blockade with dibenzyline prevented the GSR produced by endotoxin in rats , whether pregnant , diabetic , or having a unilateral ureteral occlusion , and the classic reaction in rabbits , but not that produced in renal-hypertensive rats .
	manualset3
221986	7	420749	7	NULL	NULL	0	NULL	unilateral ureteral occlusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Alpha-adrenergic blockade with dibenzyline prevented the GSR produced by endotoxin in rats , whether pregnant , diabetic , or having a unilateral ureteral occlusion , and the classic reaction in rabbits , but not that produced in renal-hypertensive rats .
	manualset3
221987	8	420749	7	NULL	NULL	0	NULL	classic reaction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Alpha-adrenergic blockade with dibenzyline prevented the GSR produced by endotoxin in rats , whether pregnant , diabetic , or having a unilateral ureteral occlusion , and the classic reaction in rabbits , but not that produced in renal-hypertensive rats .
	manualset3
221988	9	420749	7	NULL	NULL	0	NULL	rabbits	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Alpha-adrenergic blockade with dibenzyline prevented the GSR produced by endotoxin in rats , whether pregnant , diabetic , or having a unilateral ureteral occlusion , and the classic reaction in rabbits , but not that produced in renal-hypertensive rats .
	manualset3
221989	10	420749	7	NULL	NULL	0	NULL	renal-hypertensive rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Alpha-adrenergic blockade with dibenzyline prevented the GSR produced by endotoxin in rats , whether pregnant , diabetic , or having a unilateral ureteral occlusion , and the classic reaction in rabbits , but not that produced in renal-hypertensive rats .
	manualset3
221990	1	420750	7	NULL	NULL	0	NULL	Structural surface changes 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural surface changes and inflammatory responses against alginate-based microcapsules after exposure to human peritoneal fluid .
	manualset3
221991	2	420750	7	NULL	NULL	0	NULL	inflammatory responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural surface changes and inflammatory responses against alginate-based microcapsules after exposure to human peritoneal fluid .
	manualset3
221992	3	420750	7	NULL	NULL	0	NULL	alginate-based microcapsules	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural surface changes and inflammatory responses against alginate-based microcapsules after exposure to human peritoneal fluid .
	manualset3
221993	4	420750	7	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural surface changes and inflammatory responses against alginate-based microcapsules after exposure to human peritoneal fluid .
	manualset3
221994	5	420750	7	NULL	NULL	0	NULL	human peritoneal fluid	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Structural surface changes and inflammatory responses against alginate-based microcapsules after exposure to human peritoneal fluid .
	manualset3
221995	1	420751	7	NULL	NULL	0	NULL	Closed scaling	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Closed scaling and root planing has limitations as a definitive procedure for the removal of calculus from deep pockets and surgical treatment may be indicated for nonresponding sites .
	manualset3
221996	2	420751	7	NULL	NULL	0	NULL	root planing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Closed scaling and root planing has limitations as a definitive procedure for the removal of calculus from deep pockets and surgical treatment may be indicated for nonresponding sites .
	manualset3
221997	3	420751	7	NULL	NULL	0	NULL	limitations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Closed scaling and root planing has limitations as a definitive procedure for the removal of calculus from deep pockets and surgical treatment may be indicated for nonresponding sites .
	manualset3
221998	4	420751	7	NULL	NULL	0	NULL	definitive procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Closed scaling and root planing has limitations as a definitive procedure for the removal of calculus from deep pockets and surgical treatment may be indicated for nonresponding sites .
	manualset3
221999	5	420751	7	NULL	NULL	0	NULL	removal	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Closed scaling and root planing has limitations as a definitive procedure for the removal of calculus from deep pockets and surgical treatment may be indicated for nonresponding sites .
	manualset3
222000	6	420751	7	NULL	NULL	0	NULL	calculus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Closed scaling and root planing has limitations as a definitive procedure for the removal of calculus from deep pockets and surgical treatment may be indicated for nonresponding sites .
	manualset3
222001	7	420751	7	NULL	NULL	0	NULL	 deep pockets 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Closed scaling and root planing has limitations as a definitive procedure for the removal of calculus from deep pockets and surgical treatment may be indicated for nonresponding sites .
	manualset3
222002	8	420751	7	NULL	NULL	0	NULL	surgical treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Closed scaling and root planing has limitations as a definitive procedure for the removal of calculus from deep pockets and surgical treatment may be indicated for nonresponding sites .
	manualset3
222003	9	420751	7	NULL	NULL	0	NULL	nonresponding sites	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Closed scaling and root planing has limitations as a definitive procedure for the removal of calculus from deep pockets and surgical treatment may be indicated for nonresponding sites .
	manualset3
222004	1	420752	7	NULL	NULL	0	NULL	 family planning services	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Where family planning services are denied or restricted , women , but not men , are denied the right to medically protect their lives and health against danger .
	manualset3
222005	2	420752	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Where family planning services are denied or restricted , women , but not men , are denied the right to medically protect their lives and health against danger .
	manualset3
222006	3	420752	7	NULL	NULL	0	NULL	 men 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Where family planning services are denied or restricted , women , but not men , are denied the right to medically protect their lives and health against danger .
	manualset3
222007	4	420752	7	NULL	NULL	0	NULL	lives	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Where family planning services are denied or restricted , women , but not men , are denied the right to medically protect their lives and health against danger .
	manualset3
222008	5	420752	7	NULL	NULL	0	NULL	health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Where family planning services are denied or restricted , women , but not men , are denied the right to medically protect their lives and health against danger .
	manualset3
222009	6	420752	7	NULL	NULL	0	NULL	 danger	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Where family planning services are denied or restricted , women , but not men , are denied the right to medically protect their lives and health against danger .
	manualset3
222010	1	420753	7	NULL	NULL	0	NULL	diabetics	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among diabetics , the AR/beta-actin R was higher in group III ( 0.088 ; CI , 0.068-0 .108 ) than in group I ( 0.045 ; CI , 0.033-0 .057 ; P & lt ; 0.01 ) .
	manualset3
222011	2	420753	7	NULL	NULL	0	NULL	AR/beta-actin R	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among diabetics , the AR/beta-actin R was higher in group III ( 0.088 ; CI , 0.068-0 .108 ) than in group I ( 0.045 ; CI , 0.033-0 .057 ; P & lt ; 0.01 ) .
	manualset3
222012	3	420753	7	NULL	NULL	0	NULL	group III	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among diabetics , the AR/beta-actin R was higher in group III ( 0.088 ; CI , 0.068-0 .108 ) than in group I ( 0.045 ; CI , 0.033-0 .057 ; P & lt ; 0.01 ) .
	manualset3
222013	4	420753	7	NULL	NULL	0	NULL	0.088	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Among diabetics , the AR/beta-actin R was higher in group III ( 0.088 ; CI , 0.068-0 .108 ) than in group I ( 0.045 ; CI , 0.033-0 .057 ; P & lt ; 0.01 ) .
	manualset3
222014	5	420753	7	NULL	NULL	0	NULL	CI , 0.068-0 .108 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among diabetics , the AR/beta-actin R was higher in group III ( 0.088 ; CI , 0.068-0 .108 ) than in group I ( 0.045 ; CI , 0.033-0 .057 ; P & lt ; 0.01 ) .
	manualset3
222015	6	420753	7	NULL	NULL	0	NULL	group I 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among diabetics , the AR/beta-actin R was higher in group III ( 0.088 ; CI , 0.068-0 .108 ) than in group I ( 0.045 ; CI , 0.033-0 .057 ; P & lt ; 0.01 ) .
	manualset3
222016	7	420753	7	NULL	NULL	0	NULL	0.045	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Among diabetics , the AR/beta-actin R was higher in group III ( 0.088 ; CI , 0.068-0 .108 ) than in group I ( 0.045 ; CI , 0.033-0 .057 ; P & lt ; 0.01 ) .
	manualset3
222017	8	420753	7	NULL	NULL	0	NULL	CI , 0.033-0 .057	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among diabetics , the AR/beta-actin R was higher in group III ( 0.088 ; CI , 0.068-0 .108 ) than in group I ( 0.045 ; CI , 0.033-0 .057 ; P & lt ; 0.01 ) .
	manualset3
222018	9	420753	7	NULL	NULL	0	NULL	P & lt ; 0.01	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among diabetics , the AR/beta-actin R was higher in group III ( 0.088 ; CI , 0.068-0 .108 ) than in group I ( 0.045 ; CI , 0.033-0 .057 ; P & lt ; 0.01 ) .
	manualset3
222019	1	420754	7	NULL	NULL	0	NULL	High speed optically sectioned fluorescence lifetime imaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	High speed optically sectioned fluorescence lifetime imaging permits study of live cell signaling events .
	manualset3
222020	2	420754	7	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	High speed optically sectioned fluorescence lifetime imaging permits study of live cell signaling events .
	manualset3
222021	3	420754	7	NULL	NULL	0	NULL	live cell signaling events	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	High speed optically sectioned fluorescence lifetime imaging permits study of live cell signaling events .
	manualset3
222022	1	420755	7	NULL	NULL	0	NULL	Inter-endoscopist variation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inter-endoscopist variation in polyp and neoplasia pick-up rates in flexible sigmoidoscopy screening for colorectal cancer .
	manualset3
222023	2	420755	7	NULL	NULL	0	NULL	polyp	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Inter-endoscopist variation in polyp and neoplasia pick-up rates in flexible sigmoidoscopy screening for colorectal cancer .
	manualset3
222024	3	420755	7	NULL	NULL	0	NULL	neoplasia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Inter-endoscopist variation in polyp and neoplasia pick-up rates in flexible sigmoidoscopy screening for colorectal cancer .
	manualset3
222025	4	420755	7	NULL	NULL	0	NULL	pick-up rates	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inter-endoscopist variation in polyp and neoplasia pick-up rates in flexible sigmoidoscopy screening for colorectal cancer .
	manualset3
222026	5	420755	7	NULL	NULL	0	NULL	 flexible sigmoidoscopy screening	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Inter-endoscopist variation in polyp and neoplasia pick-up rates in flexible sigmoidoscopy screening for colorectal cancer .
	manualset3
222027	6	420755	7	NULL	NULL	0	NULL	 colorectal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Inter-endoscopist variation in polyp and neoplasia pick-up rates in flexible sigmoidoscopy screening for colorectal cancer .
	manualset3
222028	1	420756	7	NULL	NULL	0	NULL	Statistical correlations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistical correlations were made among prednisolone ( PRED ) and/or dexamethasone ( DEX ) LCS50 and absolute number of blast cells ( ANB ) on day 0/8 and a new parameter named blast cells clearance ( BCC , BCC8 ( % ) = ANB8 : ANB0 x 100 ) on day 8 .
	manualset3
222029	2	420756	7	NULL	NULL	0	NULL	prednisolone ( PRED )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistical correlations were made among prednisolone ( PRED ) and/or dexamethasone ( DEX ) LCS50 and absolute number of blast cells ( ANB ) on day 0/8 and a new parameter named blast cells clearance ( BCC , BCC8 ( % ) = ANB8 : ANB0 x 100 ) on day 8 .
	manualset3
222030	3	420756	7	NULL	NULL	NULL	NULL	dexamethasone ( DEX ) LCS50 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Statistical correlations were made among prednisolone ( PRED ) and/or dexamethasone ( DEX ) LCS50 and absolute number of blast cells ( ANB ) on day 0/8 and a new parameter named blast cells clearance ( BCC , BCC8 ( % ) = ANB8 : ANB0 x 100 ) on day 8 .
	manualset3
222031	4	420756	7	NULL	NULL	0	NULL	absolute number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistical correlations were made among prednisolone ( PRED ) and/or dexamethasone ( DEX ) LCS50 and absolute number of blast cells ( ANB ) on day 0/8 and a new parameter named blast cells clearance ( BCC , BCC8 ( % ) = ANB8 : ANB0 x 100 ) on day 8 .
	manualset3
222032	5	420756	7	NULL	NULL	0	NULL	blast cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistical correlations were made among prednisolone ( PRED ) and/or dexamethasone ( DEX ) LCS50 and absolute number of blast cells ( ANB ) on day 0/8 and a new parameter named blast cells clearance ( BCC , BCC8 ( % ) = ANB8 : ANB0 x 100 ) on day 8 .
	manualset3
222033	6	420756	7	NULL	NULL	0	NULL	ANB	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistical correlations were made among prednisolone ( PRED ) and/or dexamethasone ( DEX ) LCS50 and absolute number of blast cells ( ANB ) on day 0/8 and a new parameter named blast cells clearance ( BCC , BCC8 ( % ) = ANB8 : ANB0 x 100 ) on day 8 .
	manualset3
222034	7	420756	7	NULL	NULL	0	NULL	day 0/8	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistical correlations were made among prednisolone ( PRED ) and/or dexamethasone ( DEX ) LCS50 and absolute number of blast cells ( ANB ) on day 0/8 and a new parameter named blast cells clearance ( BCC , BCC8 ( % ) = ANB8 : ANB0 x 100 ) on day 8 .
	manualset3
222035	8	420756	7	NULL	NULL	0	NULL	new parameter	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistical correlations were made among prednisolone ( PRED ) and/or dexamethasone ( DEX ) LCS50 and absolute number of blast cells ( ANB ) on day 0/8 and a new parameter named blast cells clearance ( BCC , BCC8 ( % ) = ANB8 : ANB0 x 100 ) on day 8 .
	manualset3
222036	9	420756	7	NULL	NULL	0	NULL	blast cells clearance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistical correlations were made among prednisolone ( PRED ) and/or dexamethasone ( DEX ) LCS50 and absolute number of blast cells ( ANB ) on day 0/8 and a new parameter named blast cells clearance ( BCC , BCC8 ( % ) = ANB8 : ANB0 x 100 ) on day 8 .
	manualset3
222037	10	420756	7	NULL	NULL	0	NULL	BCC 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistical correlations were made among prednisolone ( PRED ) and/or dexamethasone ( DEX ) LCS50 and absolute number of blast cells ( ANB ) on day 0/8 and a new parameter named blast cells clearance ( BCC , BCC8 ( % ) = ANB8 : ANB0 x 100 ) on day 8 .
	manualset3
222038	11	420756	7	NULL	NULL	0	NULL	BCC8 ( % ) = ANB8 : ANB0 x 100	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistical correlations were made among prednisolone ( PRED ) and/or dexamethasone ( DEX ) LCS50 and absolute number of blast cells ( ANB ) on day 0/8 and a new parameter named blast cells clearance ( BCC , BCC8 ( % ) = ANB8 : ANB0 x 100 ) on day 8 .
	manualset3
222039	12	420756	7	NULL	NULL	0	NULL	 day 8	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistical correlations were made among prednisolone ( PRED ) and/or dexamethasone ( DEX ) LCS50 and absolute number of blast cells ( ANB ) on day 0/8 and a new parameter named blast cells clearance ( BCC , BCC8 ( % ) = ANB8 : ANB0 x 100 ) on day 8 .
	manualset3
222040	1	420757	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the level of phosphocreatine is roughly 10-times higher compared to ATP .
	manualset3
222041	2	420757	7	NULL	NULL	0	NULL	level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the level of phosphocreatine is roughly 10-times higher compared to ATP .
	manualset3
222042	3	420757	7	NULL	NULL	0	NULL	 phosphocreatine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the level of phosphocreatine is roughly 10-times higher compared to ATP .
	manualset3
222043	4	420757	7	NULL	NULL	0	NULL	10-times	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the level of phosphocreatine is roughly 10-times higher compared to ATP .
	manualset3
222044	5	420757	7	NULL	NULL	0	NULL	ATP 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the level of phosphocreatine is roughly 10-times higher compared to ATP .
	manualset3
222045	1	420758	7	NULL	NULL	0	NULL	High temperature stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( High temperature stress on rice anthesis : research progress and prospects ) .
	manualset3
222046	2	420758	7	NULL	NULL	NULL	NULL	rice anthesis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( High temperature stress on rice anthesis : research progress and prospects ) .
	manualset3
222047	3	420758	7	NULL	NULL	0	NULL	research progress 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( High temperature stress on rice anthesis : research progress and prospects ) .
	manualset3
222048	4	420758	7	NULL	NULL	0	NULL	prospects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( High temperature stress on rice anthesis : research progress and prospects ) .
	manualset3
222049	1	420759	7	NULL	NULL	0	NULL	dialysis patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among dialysis patients little risk reduction appears to be achieved by treatment of low-density lipoprotein cholesterol level .
	manualset3
222050	2	420759	7	NULL	NULL	0	NULL	 little risk reduction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among dialysis patients little risk reduction appears to be achieved by treatment of low-density lipoprotein cholesterol level .
	manualset3
222051	3	420759	7	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Among dialysis patients little risk reduction appears to be achieved by treatment of low-density lipoprotein cholesterol level .
	manualset3
222052	4	420759	7	NULL	NULL	0	NULL	low-density lipoprotein cholesterol level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among dialysis patients little risk reduction appears to be achieved by treatment of low-density lipoprotein cholesterol level .
	manualset3
222053	1	420760	7	NULL	NULL	0	NULL	Long-term results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term results of chemoradiotherapy for locally advanced esophageal cancer , using daily low-dose 5-fluorouracil and cis-diammine-dichloro-platinum ( CDDP ) .
	manualset3
222054	2	420760	7	NULL	NULL	0	NULL	chemoradiotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term results of chemoradiotherapy for locally advanced esophageal cancer , using daily low-dose 5-fluorouracil and cis-diammine-dichloro-platinum ( CDDP ) .
	manualset3
222055	3	420760	7	NULL	NULL	0	NULL	locally advanced esophageal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term results of chemoradiotherapy for locally advanced esophageal cancer , using daily low-dose 5-fluorouracil and cis-diammine-dichloro-platinum ( CDDP ) .
	manualset3
222056	4	420760	7	NULL	NULL	0	NULL	 daily low-dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term results of chemoradiotherapy for locally advanced esophageal cancer , using daily low-dose 5-fluorouracil and cis-diammine-dichloro-platinum ( CDDP ) .
	manualset3
222057	5	420760	7	NULL	NULL	0	NULL	5-fluorouracil 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term results of chemoradiotherapy for locally advanced esophageal cancer , using daily low-dose 5-fluorouracil and cis-diammine-dichloro-platinum ( CDDP ) .
	manualset3
222058	6	420760	7	NULL	NULL	0	NULL	cis-diammine-dichloro-platinum ( CDDP ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term results of chemoradiotherapy for locally advanced esophageal cancer , using daily low-dose 5-fluorouracil and cis-diammine-dichloro-platinum ( CDDP ) .
	manualset3
222365	1	420761	7	NULL	NULL	0	NULL	Cardiac myocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Cardiac myocytes are the primary site of GRP78 expression within the heart .
	manualset3
222366	2	420761	7	NULL	NULL	0	NULL	primary site	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Cardiac myocytes are the primary site of GRP78 expression within the heart .
	manualset3
222367	3	420761	7	NULL	NULL	0	NULL	GRP78 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cardiac myocytes are the primary site of GRP78 expression within the heart .
	manualset3
222368	4	420761	7	NULL	NULL	0	NULL	heart	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Cardiac myocytes are the primary site of GRP78 expression within the heart .
	manualset3
222369	1	420762	7	NULL	NULL	0	NULL	Incorporation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of 14C-glycine into heme was 45 % less in senescent rat marrow cells , whereas incorporation of 14C-delta-aminolevulinic acid was not related to age .
	manualset3
222370	2	420762	7	NULL	NULL	0	NULL	14C-glycine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of 14C-glycine into heme was 45 % less in senescent rat marrow cells , whereas incorporation of 14C-delta-aminolevulinic acid was not related to age .
	manualset3
222371	3	420762	7	NULL	NULL	0	NULL	heme	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of 14C-glycine into heme was 45 % less in senescent rat marrow cells , whereas incorporation of 14C-delta-aminolevulinic acid was not related to age .
	manualset3
222372	4	420762	7	NULL	NULL	0	NULL	45 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of 14C-glycine into heme was 45 % less in senescent rat marrow cells , whereas incorporation of 14C-delta-aminolevulinic acid was not related to age .
	manualset3
222373	5	420762	7	NULL	NULL	0	NULL	senescent rat marrow cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of 14C-glycine into heme was 45 % less in senescent rat marrow cells , whereas incorporation of 14C-delta-aminolevulinic acid was not related to age .
	manualset3
222374	6	420762	7	NULL	NULL	0	NULL	 incorporation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of 14C-glycine into heme was 45 % less in senescent rat marrow cells , whereas incorporation of 14C-delta-aminolevulinic acid was not related to age .
	manualset3
222375	7	420762	7	NULL	NULL	0	NULL	14C-delta-aminolevulinic acid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of 14C-glycine into heme was 45 % less in senescent rat marrow cells , whereas incorporation of 14C-delta-aminolevulinic acid was not related to age .
	manualset3
222376	8	420762	7	NULL	NULL	0	NULL	age	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Incorporation of 14C-glycine into heme was 45 % less in senescent rat marrow cells , whereas incorporation of 14C-delta-aminolevulinic acid was not related to age .
	manualset3
222377	1	420763	7	NULL	NULL	0	NULL	Understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Understanding the biology and immunopathology of HIV-1 early following infection , its modes of transmission and the human immune system 's response to the virus should aid in the rational design of vaccines of increased efficacy .
	manualset3
222378	2	420763	7	NULL	NULL	0	NULL	biology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Understanding the biology and immunopathology of HIV-1 early following infection , its modes of transmission and the human immune system 's response to the virus should aid in the rational design of vaccines of increased efficacy .
	manualset3
222379	3	420763	7	NULL	NULL	0	NULL	immunopathology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Understanding the biology and immunopathology of HIV-1 early following infection , its modes of transmission and the human immune system 's response to the virus should aid in the rational design of vaccines of increased efficacy .
	manualset3
222380	4	420763	7	NULL	NULL	0	NULL	HIV-1 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Understanding the biology and immunopathology of HIV-1 early following infection , its modes of transmission and the human immune system 's response to the virus should aid in the rational design of vaccines of increased efficacy .
	manualset3
222381	5	420763	7	NULL	NULL	0	NULL	infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Understanding the biology and immunopathology of HIV-1 early following infection , its modes of transmission and the human immune system 's response to the virus should aid in the rational design of vaccines of increased efficacy .
	manualset3
222382	6	420763	7	NULL	NULL	0	NULL	modes of transmission 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Understanding the biology and immunopathology of HIV-1 early following infection , its modes of transmission and the human immune system 's response to the virus should aid in the rational design of vaccines of increased efficacy .
	manualset3
222383	7	420763	7	NULL	NULL	0	NULL	human immune system 's response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Understanding the biology and immunopathology of HIV-1 early following infection , its modes of transmission and the human immune system 's response to the virus should aid in the rational design of vaccines of increased efficacy .
	manualset3
222384	8	420763	7	NULL	NULL	0	NULL	virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Understanding the biology and immunopathology of HIV-1 early following infection , its modes of transmission and the human immune system 's response to the virus should aid in the rational design of vaccines of increased efficacy .
	manualset3
222385	9	420763	7	NULL	NULL	0	NULL	rational design	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Understanding the biology and immunopathology of HIV-1 early following infection , its modes of transmission and the human immune system 's response to the virus should aid in the rational design of vaccines of increased efficacy .
	manualset3
222386	10	420763	7	NULL	NULL	0	NULL	vaccines 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Understanding the biology and immunopathology of HIV-1 early following infection , its modes of transmission and the human immune system 's response to the virus should aid in the rational design of vaccines of increased efficacy .
	manualset3
222387	11	420763	7	NULL	NULL	0	NULL	increased efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Understanding the biology and immunopathology of HIV-1 early following infection , its modes of transmission and the human immune system 's response to the virus should aid in the rational design of vaccines of increased efficacy .
	manualset3
222388	1	420764	7	NULL	NULL	0	NULL	experimental results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent experimental results by Linden showed that monocular lid suture and monocular inactivation do not change the mean firing rates of LGN neurons but that lid suture reduces correlations between adjacent neurons whereas monocular inactivation leads to correlated firing .
	manualset3
222389	2	420764	7	NULL	NULL	0	NULL	Linden	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent experimental results by Linden showed that monocular lid suture and monocular inactivation do not change the mean firing rates of LGN neurons but that lid suture reduces correlations between adjacent neurons whereas monocular inactivation leads to correlated firing .
	manualset3
222390	3	420764	7	NULL	NULL	0	NULL	monocular lid suture	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent experimental results by Linden showed that monocular lid suture and monocular inactivation do not change the mean firing rates of LGN neurons but that lid suture reduces correlations between adjacent neurons whereas monocular inactivation leads to correlated firing .
	manualset3
222391	4	420764	7	NULL	NULL	0	NULL	monocular inactivation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent experimental results by Linden showed that monocular lid suture and monocular inactivation do not change the mean firing rates of LGN neurons but that lid suture reduces correlations between adjacent neurons whereas monocular inactivation leads to correlated firing .
	manualset3
222392	5	420764	7	NULL	NULL	0	NULL	mean firing rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent experimental results by Linden showed that monocular lid suture and monocular inactivation do not change the mean firing rates of LGN neurons but that lid suture reduces correlations between adjacent neurons whereas monocular inactivation leads to correlated firing .
	manualset3
222393	6	420764	7	NULL	NULL	0	NULL	LGN neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent experimental results by Linden showed that monocular lid suture and monocular inactivation do not change the mean firing rates of LGN neurons but that lid suture reduces correlations between adjacent neurons whereas monocular inactivation leads to correlated firing .
	manualset3
222394	7	420764	7	NULL	NULL	0	NULL	lid suture	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent experimental results by Linden showed that monocular lid suture and monocular inactivation do not change the mean firing rates of LGN neurons but that lid suture reduces correlations between adjacent neurons whereas monocular inactivation leads to correlated firing .
	manualset3
222395	8	420764	7	NULL	NULL	0	NULL	correlations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent experimental results by Linden showed that monocular lid suture and monocular inactivation do not change the mean firing rates of LGN neurons but that lid suture reduces correlations between adjacent neurons whereas monocular inactivation leads to correlated firing .
	manualset3
222396	9	420764	7	NULL	NULL	0	NULL	adjacent neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent experimental results by Linden showed that monocular lid suture and monocular inactivation do not change the mean firing rates of LGN neurons but that lid suture reduces correlations between adjacent neurons whereas monocular inactivation leads to correlated firing .
	manualset3
222397	10	420764	7	NULL	NULL	0	NULL	monocular inactivation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent experimental results by Linden showed that monocular lid suture and monocular inactivation do not change the mean firing rates of LGN neurons but that lid suture reduces correlations between adjacent neurons whereas monocular inactivation leads to correlated firing .
	manualset3
222398	11	420764	7	NULL	NULL	0	NULL	correlated firing 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent experimental results by Linden showed that monocular lid suture and monocular inactivation do not change the mean firing rates of LGN neurons but that lid suture reduces correlations between adjacent neurons whereas monocular inactivation leads to correlated firing .
	manualset3
222399	1	420765	7	NULL	NULL	0	NULL	Redox control	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Redox control of a polymerization catalyst by changing the oxidation state of the metal center .
	manualset3
222400	2	420765	7	NULL	NULL	0	NULL	polymerization catalyst	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Redox control of a polymerization catalyst by changing the oxidation state of the metal center .
	manualset3
222401	3	420765	7	NULL	NULL	0	NULL	oxidation state	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Redox control of a polymerization catalyst by changing the oxidation state of the metal center .
	manualset3
222402	4	420765	7	NULL	NULL	0	NULL	 metal center	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Redox control of a polymerization catalyst by changing the oxidation state of the metal center .
	manualset3
222403	1	420766	7	NULL	NULL	0	NULL	3-year treatment period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	During the 3-year treatment period , participants received a daily supplement containing either placebo , or calcium , magnesium , zinc , and vitamin D ( MD group ) , or the same formulation with additional vitamin K1 ( MDK group ) .
	manualset3
222404	2	420766	7	NULL	NULL	0	NULL	participants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	During the 3-year treatment period , participants received a daily supplement containing either placebo , or calcium , magnesium , zinc , and vitamin D ( MD group ) , or the same formulation with additional vitamin K1 ( MDK group ) .
	manualset3
222405	3	420766	7	NULL	NULL	0	NULL	daily supplement 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	During the 3-year treatment period , participants received a daily supplement containing either placebo , or calcium , magnesium , zinc , and vitamin D ( MD group ) , or the same formulation with additional vitamin K1 ( MDK group ) .
	manualset3
222406	4	420766	7	NULL	NULL	0	NULL	placebo 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	During the 3-year treatment period , participants received a daily supplement containing either placebo , or calcium , magnesium , zinc , and vitamin D ( MD group ) , or the same formulation with additional vitamin K1 ( MDK group ) .
	manualset3
222407	5	420766	7	NULL	NULL	0	NULL	calcium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	During the 3-year treatment period , participants received a daily supplement containing either placebo , or calcium , magnesium , zinc , and vitamin D ( MD group ) , or the same formulation with additional vitamin K1 ( MDK group ) .
	manualset3
222408	6	420766	7	NULL	NULL	0	NULL	magnesium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	During the 3-year treatment period , participants received a daily supplement containing either placebo , or calcium , magnesium , zinc , and vitamin D ( MD group ) , or the same formulation with additional vitamin K1 ( MDK group ) .
	manualset3
222409	7	420766	7	NULL	NULL	0	NULL	 zinc	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	During the 3-year treatment period , participants received a daily supplement containing either placebo , or calcium , magnesium , zinc , and vitamin D ( MD group ) , or the same formulation with additional vitamin K1 ( MDK group ) .
	manualset3
222410	8	420766	7	NULL	NULL	0	NULL	vitamin D ( MD group )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	During the 3-year treatment period , participants received a daily supplement containing either placebo , or calcium , magnesium , zinc , and vitamin D ( MD group ) , or the same formulation with additional vitamin K1 ( MDK group ) .
	manualset3
222411	9	420766	7	NULL	NULL	0	NULL	formulation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	During the 3-year treatment period , participants received a daily supplement containing either placebo , or calcium , magnesium , zinc , and vitamin D ( MD group ) , or the same formulation with additional vitamin K1 ( MDK group ) .
	manualset3
222412	10	420766	7	NULL	NULL	0	NULL	vitamin K1 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	During the 3-year treatment period , participants received a daily supplement containing either placebo , or calcium , magnesium , zinc , and vitamin D ( MD group ) , or the same formulation with additional vitamin K1 ( MDK group ) .
	manualset3
222413	11	420766	7	NULL	NULL	0	NULL	MDK group 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	During the 3-year treatment period , participants received a daily supplement containing either placebo , or calcium , magnesium , zinc , and vitamin D ( MD group ) , or the same formulation with additional vitamin K1 ( MDK group ) .
	manualset3
222414	1	420767	7	NULL	NULL	0	NULL	early problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among early problems of the program were opposition from physicians , difficulty of recruiting volunteers who met the personality and other requirements , myths and incorrect beliefs of the community regarding family planning , the belief among men that contraception would encourage infidelity among women , and official pronatalist policies .
	manualset3
222415	2	420767	7	NULL	NULL	0	NULL	program	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Among early problems of the program were opposition from physicians , difficulty of recruiting volunteers who met the personality and other requirements , myths and incorrect beliefs of the community regarding family planning , the belief among men that contraception would encourage infidelity among women , and official pronatalist policies .
	manualset3
222416	3	420767	7	NULL	NULL	0	NULL	physicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among early problems of the program were opposition from physicians , difficulty of recruiting volunteers who met the personality and other requirements , myths and incorrect beliefs of the community regarding family planning , the belief among men that contraception would encourage infidelity among women , and official pronatalist policies .
	manualset3
222417	4	420767	7	NULL	NULL	0	NULL	volunteers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among early problems of the program were opposition from physicians , difficulty of recruiting volunteers who met the personality and other requirements , myths and incorrect beliefs of the community regarding family planning , the belief among men that contraception would encourage infidelity among women , and official pronatalist policies .
	manualset3
222418	5	420767	7	NULL	NULL	0	NULL	personality	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among early problems of the program were opposition from physicians , difficulty of recruiting volunteers who met the personality and other requirements , myths and incorrect beliefs of the community regarding family planning , the belief among men that contraception would encourage infidelity among women , and official pronatalist policies .
	manualset3
222419	6	420767	7	NULL	NULL	0	NULL	requirements	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among early problems of the program were opposition from physicians , difficulty of recruiting volunteers who met the personality and other requirements , myths and incorrect beliefs of the community regarding family planning , the belief among men that contraception would encourage infidelity among women , and official pronatalist policies .
	manualset3
222420	7	420767	7	NULL	NULL	0	NULL	myths	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among early problems of the program were opposition from physicians , difficulty of recruiting volunteers who met the personality and other requirements , myths and incorrect beliefs of the community regarding family planning , the belief among men that contraception would encourage infidelity among women , and official pronatalist policies .
	manualset3
222421	8	420767	7	NULL	NULL	0	NULL	 incorrect beliefs	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among early problems of the program were opposition from physicians , difficulty of recruiting volunteers who met the personality and other requirements , myths and incorrect beliefs of the community regarding family planning , the belief among men that contraception would encourage infidelity among women , and official pronatalist policies .
	manualset3
222422	9	420767	7	NULL	NULL	0	NULL	community	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among early problems of the program were opposition from physicians , difficulty of recruiting volunteers who met the personality and other requirements , myths and incorrect beliefs of the community regarding family planning , the belief among men that contraception would encourage infidelity among women , and official pronatalist policies .
	manualset3
222423	10	420767	7	NULL	NULL	0	NULL	family planning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among early problems of the program were opposition from physicians , difficulty of recruiting volunteers who met the personality and other requirements , myths and incorrect beliefs of the community regarding family planning , the belief among men that contraception would encourage infidelity among women , and official pronatalist policies .
	manualset3
222424	11	420767	7	NULL	NULL	0	NULL	belief	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among early problems of the program were opposition from physicians , difficulty of recruiting volunteers who met the personality and other requirements , myths and incorrect beliefs of the community regarding family planning , the belief among men that contraception would encourage infidelity among women , and official pronatalist policies .
	manualset3
222425	12	420767	7	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among early problems of the program were opposition from physicians , difficulty of recruiting volunteers who met the personality and other requirements , myths and incorrect beliefs of the community regarding family planning , the belief among men that contraception would encourage infidelity among women , and official pronatalist policies .
	manualset3
222426	13	420767	7	NULL	NULL	0	NULL	contraception 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Among early problems of the program were opposition from physicians , difficulty of recruiting volunteers who met the personality and other requirements , myths and incorrect beliefs of the community regarding family planning , the belief among men that contraception would encourage infidelity among women , and official pronatalist policies .
	manualset3
222427	14	420767	7	NULL	NULL	0	NULL	infidelity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among early problems of the program were opposition from physicians , difficulty of recruiting volunteers who met the personality and other requirements , myths and incorrect beliefs of the community regarding family planning , the belief among men that contraception would encourage infidelity among women , and official pronatalist policies .
	manualset3
222428	15	420767	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among early problems of the program were opposition from physicians , difficulty of recruiting volunteers who met the personality and other requirements , myths and incorrect beliefs of the community regarding family planning , the belief among men that contraception would encourage infidelity among women , and official pronatalist policies .
	manualset3
222429	16	420767	7	NULL	NULL	0	NULL	pronatalist policies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among early problems of the program were opposition from physicians , difficulty of recruiting volunteers who met the personality and other requirements , myths and incorrect beliefs of the community regarding family planning , the belief among men that contraception would encourage infidelity among women , and official pronatalist policies .
	manualset3
224178	17	420767	7	NULL	NULL	0	NULL	 recruiting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among early problems of the program were opposition from physicians , difficulty of recruiting volunteers who met the personality and other requirements , myths and incorrect beliefs of the community regarding family planning , the belief among men that contraception would encourage infidelity among women , and official pronatalist policies .
	manualset3
228877	18	420767	7	NULL	NULL	0	NULL	opposition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among early problems of the program were opposition from physicians , difficulty of recruiting volunteers who met the personality and other requirements , myths and incorrect beliefs of the community regarding family planning , the belief among men that contraception would encourage infidelity among women , and official pronatalist policies .
	manualset3
228878	19	420767	7	NULL	NULL	0	NULL	difficulty	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among early problems of the program were opposition from physicians , difficulty of recruiting volunteers who met the personality and other requirements , myths and incorrect beliefs of the community regarding family planning , the belief among men that contraception would encourage infidelity among women , and official pronatalist policies .
	manualset3
222430	1	420768	7	NULL	NULL	0	NULL	Impaired fasting tolerance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Impaired fasting tolerance among Alaska native children with a common carnitine palmitoyltransferase 1A sequence variant .
	manualset3
222431	2	420768	7	NULL	NULL	0	NULL	Alaska native children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Impaired fasting tolerance among Alaska native children with a common carnitine palmitoyltransferase 1A sequence variant .
	manualset3
222432	3	420768	7	NULL	NULL	0	NULL	carnitine palmitoyltransferase 1A sequence variant	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Impaired fasting tolerance among Alaska native children with a common carnitine palmitoyltransferase 1A sequence variant .
	manualset3
222433	1	420769	7	NULL	NULL	0	NULL	SAM hgh level cobalt-60 irradiation facility	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The SAM hgh level cobalt-60 irradiation facility .
	manualset3
222434	1	420770	7	NULL	NULL	0	NULL	histological study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In additional histological study , bronchiolar epithelial methaplasia and alveolar septal thickening , which were characteristic findings in non-immunized infected mice , were not observed in mice immunized with 2 biweekly injection of about 250 HA of FV and then challenged .
	manualset3
222435	2	420770	7	NULL	NULL	0	NULL	 bronchiolar epithelial methaplasia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In additional histological study , bronchiolar epithelial methaplasia and alveolar septal thickening , which were characteristic findings in non-immunized infected mice , were not observed in mice immunized with 2 biweekly injection of about 250 HA of FV and then challenged .
	manualset3
222436	3	420770	7	NULL	NULL	0	NULL	alveolar septal thickening	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In additional histological study , bronchiolar epithelial methaplasia and alveolar septal thickening , which were characteristic findings in non-immunized infected mice , were not observed in mice immunized with 2 biweekly injection of about 250 HA of FV and then challenged .
	manualset3
222437	4	420770	7	NULL	NULL	0	NULL	characteristic findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In additional histological study , bronchiolar epithelial methaplasia and alveolar septal thickening , which were characteristic findings in non-immunized infected mice , were not observed in mice immunized with 2 biweekly injection of about 250 HA of FV and then challenged .
	manualset3
222438	5	420770	7	NULL	NULL	0	NULL	non-immunized infected mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In additional histological study , bronchiolar epithelial methaplasia and alveolar septal thickening , which were characteristic findings in non-immunized infected mice , were not observed in mice immunized with 2 biweekly injection of about 250 HA of FV and then challenged .
	manualset3
222439	6	420770	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In additional histological study , bronchiolar epithelial methaplasia and alveolar septal thickening , which were characteristic findings in non-immunized infected mice , were not observed in mice immunized with 2 biweekly injection of about 250 HA of FV and then challenged .
	manualset3
222440	7	420770	7	NULL	NULL	0	NULL	2 biweekly injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In additional histological study , bronchiolar epithelial methaplasia and alveolar septal thickening , which were characteristic findings in non-immunized infected mice , were not observed in mice immunized with 2 biweekly injection of about 250 HA of FV and then challenged .
	manualset3
222441	8	420770	7	NULL	NULL	0	NULL	250 HA of FV 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In additional histological study , bronchiolar epithelial methaplasia and alveolar septal thickening , which were characteristic findings in non-immunized infected mice , were not observed in mice immunized with 2 biweekly injection of about 250 HA of FV and then challenged .
	manualset3
222442	1	420771	7	NULL	NULL	0	NULL	Cumulative stresses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Cumulative stresses that may drive platelets beyond their activation threshold were calculated along multiple flow trajectories and collapsed into probability density functions ( PDFs ) representing the device ` thrombogenic footprint ' , indicating significantly reduced thrombogenicity for the optimized design .
	manualset3
222443	2	420771	7	NULL	NULL	0	NULL	platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Cumulative stresses that may drive platelets beyond their activation threshold were calculated along multiple flow trajectories and collapsed into probability density functions ( PDFs ) representing the device ` thrombogenic footprint ' , indicating significantly reduced thrombogenicity for the optimized design .
	manualset3
222444	3	420771	7	NULL	NULL	0	NULL	activation threshold 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Cumulative stresses that may drive platelets beyond their activation threshold were calculated along multiple flow trajectories and collapsed into probability density functions ( PDFs ) representing the device ` thrombogenic footprint ' , indicating significantly reduced thrombogenicity for the optimized design .
	manualset3
222445	4	420771	7	NULL	NULL	0	NULL	multiple flow trajectories	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Cumulative stresses that may drive platelets beyond their activation threshold were calculated along multiple flow trajectories and collapsed into probability density functions ( PDFs ) representing the device ` thrombogenic footprint ' , indicating significantly reduced thrombogenicity for the optimized design .
	manualset3
222446	5	420771	7	NULL	NULL	0	NULL	probability density functions ( PDFs ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Cumulative stresses that may drive platelets beyond their activation threshold were calculated along multiple flow trajectories and collapsed into probability density functions ( PDFs ) representing the device ` thrombogenic footprint ' , indicating significantly reduced thrombogenicity for the optimized design .
	manualset3
222447	6	420771	7	NULL	NULL	0	NULL	device	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Cumulative stresses that may drive platelets beyond their activation threshold were calculated along multiple flow trajectories and collapsed into probability density functions ( PDFs ) representing the device ` thrombogenic footprint ' , indicating significantly reduced thrombogenicity for the optimized design .
	manualset3
222448	7	420771	7	NULL	NULL	0	NULL	thrombogenic footprint 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Cumulative stresses that may drive platelets beyond their activation threshold were calculated along multiple flow trajectories and collapsed into probability density functions ( PDFs ) representing the device ` thrombogenic footprint ' , indicating significantly reduced thrombogenicity for the optimized design .
	manualset3
222449	8	420771	7	NULL	NULL	0	NULL	thrombogenicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Cumulative stresses that may drive platelets beyond their activation threshold were calculated along multiple flow trajectories and collapsed into probability density functions ( PDFs ) representing the device ` thrombogenic footprint ' , indicating significantly reduced thrombogenicity for the optimized design .
	manualset3
222450	9	420771	7	NULL	NULL	0	NULL	optimized design	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Cumulative stresses that may drive platelets beyond their activation threshold were calculated along multiple flow trajectories and collapsed into probability density functions ( PDFs ) representing the device ` thrombogenic footprint ' , indicating significantly reduced thrombogenicity for the optimized design .
	manualset3
222451	1	420772	7	NULL	NULL	0	NULL	LPS activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	LPS activation of the clone resulted in a net increase of IL-1 , IL-6 , and TNF-alpha production .
	manualset3
222452	2	420772	7	NULL	NULL	0	NULL	clone	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	LPS activation of the clone resulted in a net increase of IL-1 , IL-6 , and TNF-alpha production .
	manualset3
222453	3	420772	7	NULL	NULL	0	NULL	 IL-1 production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	LPS activation of the clone resulted in a net increase of IL-1 , IL-6 , and TNF-alpha production .
	manualset3
222454	4	420772	7	NULL	NULL	0	NULL	IL-6 production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	LPS activation of the clone resulted in a net increase of IL-1 , IL-6 , and TNF-alpha production .
	manualset3
222455	5	420772	7	NULL	NULL	0	NULL	TNF-alpha production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	LPS activation of the clone resulted in a net increase of IL-1 , IL-6 , and TNF-alpha production .
	manualset3
222456	1	420773	7	NULL	NULL	0	NULL	Cervical lymph node metastases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cervical lymph node metastases from an unknown primary tumor ) .
	manualset3
222457	2	420773	7	NULL	NULL	0	NULL	 unknown primary tumor	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Cervical lymph node metastases from an unknown primary tumor ) .
	manualset3
222458	1	420774	7	NULL	NULL	0	NULL	Multidisciplinary procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Multidisciplinary procedures were more frequent in moderately and severely affected NF1 patients than in milder cases ( P & lt ; 0 .
	manualset3
222459	2	420774	7	NULL	NULL	0	NULL	NF1 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Multidisciplinary procedures were more frequent in moderately and severely affected NF1 patients than in milder cases ( P & lt ; 0 .
	manualset3
222460	3	420774	7	NULL	NULL	0	NULL	milder cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Multidisciplinary procedures were more frequent in moderately and severely affected NF1 patients than in milder cases ( P & lt ; 0 .
	manualset3
222461	4	420774	7	NULL	NULL	0	NULL	P & lt ; 0	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Multidisciplinary procedures were more frequent in moderately and severely affected NF1 patients than in milder cases ( P & lt ; 0 .
	manualset3
222462	1	420775	7	NULL	NULL	0	NULL	multiple ETS transcripts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Among multiple ETS transcripts present , ETS1 , FLI1 , ETV1 , ETV5 , ERG , and ETV6 were the most abundant in the early embryonic heart .
	manualset3
222463	2	420775	7	NULL	NULL	0	NULL	ETS1	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Among multiple ETS transcripts present , ETS1 , FLI1 , ETV1 , ETV5 , ERG , and ETV6 were the most abundant in the early embryonic heart .
	manualset3
222464	3	420775	7	NULL	NULL	0	NULL	FLI1	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Among multiple ETS transcripts present , ETS1 , FLI1 , ETV1 , ETV5 , ERG , and ETV6 were the most abundant in the early embryonic heart .
	manualset3
222465	4	420775	7	NULL	NULL	0	NULL	ETV1	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Among multiple ETS transcripts present , ETS1 , FLI1 , ETV1 , ETV5 , ERG , and ETV6 were the most abundant in the early embryonic heart .
	manualset3
222466	5	420775	7	NULL	NULL	0	NULL	ETV5	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Among multiple ETS transcripts present , ETS1 , FLI1 , ETV1 , ETV5 , ERG , and ETV6 were the most abundant in the early embryonic heart .
	manualset3
222467	6	420775	7	NULL	NULL	0	NULL	ERG	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Among multiple ETS transcripts present , ETS1 , FLI1 , ETV1 , ETV5 , ERG , and ETV6 were the most abundant in the early embryonic heart .
	manualset3
222468	7	420775	7	NULL	NULL	0	NULL	ETV6	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Among multiple ETS transcripts present , ETS1 , FLI1 , ETV1 , ETV5 , ERG , and ETV6 were the most abundant in the early embryonic heart .
	manualset3
222469	8	420775	7	NULL	NULL	0	NULL	early embryonic heart	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Among multiple ETS transcripts present , ETS1 , FLI1 , ETV1 , ETV5 , ERG , and ETV6 were the most abundant in the early embryonic heart .
	manualset3
222470	1	420776	7	NULL	NULL	0	NULL	cultured heart cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In cultured heart cells , the amount of CO2 obtained from the carboxyl group was much higher than that obtained from the methyl group .
	manualset3
222471	2	420776	7	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In cultured heart cells , the amount of CO2 obtained from the carboxyl group was much higher than that obtained from the methyl group .
	manualset3
222472	3	420776	7	NULL	NULL	0	NULL	CO2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In cultured heart cells , the amount of CO2 obtained from the carboxyl group was much higher than that obtained from the methyl group .
	manualset3
222473	4	420776	7	NULL	NULL	0	NULL	carboxyl group	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In cultured heart cells , the amount of CO2 obtained from the carboxyl group was much higher than that obtained from the methyl group .
	manualset3
222474	5	420776	7	NULL	NULL	0	NULL	methyl group	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In cultured heart cells , the amount of CO2 obtained from the carboxyl group was much higher than that obtained from the methyl group .
	manualset3
222475	1	420777	7	NULL	NULL	0	NULL	NEW OPIOID ANALGESICS 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	NEW OPIOID ANALGESICS : Progress in pain reliet has recently been achieved with the introduction of new opioid analgesics such as tramadol and the pediatric preparation of codeine phosphate as well as powerful long-release opioids which can be administered per os , or percutaneously for transdermal fentanyl .
	manualset3
222476	2	420777	7	NULL	NULL	0	NULL	Progress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	NEW OPIOID ANALGESICS : Progress in pain reliet has recently been achieved with the introduction of new opioid analgesics such as tramadol and the pediatric preparation of codeine phosphate as well as powerful long-release opioids which can be administered per os , or percutaneously for transdermal fentanyl .
	manualset3
222477	3	420777	7	NULL	NULL	0	NULL	pain reliet	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	NEW OPIOID ANALGESICS : Progress in pain reliet has recently been achieved with the introduction of new opioid analgesics such as tramadol and the pediatric preparation of codeine phosphate as well as powerful long-release opioids which can be administered per os , or percutaneously for transdermal fentanyl .
	manualset3
222478	4	420777	7	NULL	NULL	0	NULL	introduction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	NEW OPIOID ANALGESICS : Progress in pain reliet has recently been achieved with the introduction of new opioid analgesics such as tramadol and the pediatric preparation of codeine phosphate as well as powerful long-release opioids which can be administered per os , or percutaneously for transdermal fentanyl .
	manualset3
222479	5	420777	7	NULL	NULL	0	NULL	new opioid analgesics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	NEW OPIOID ANALGESICS : Progress in pain reliet has recently been achieved with the introduction of new opioid analgesics such as tramadol and the pediatric preparation of codeine phosphate as well as powerful long-release opioids which can be administered per os , or percutaneously for transdermal fentanyl .
	manualset3
222480	6	420777	7	NULL	NULL	0	NULL	tramadol 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	NEW OPIOID ANALGESICS : Progress in pain reliet has recently been achieved with the introduction of new opioid analgesics such as tramadol and the pediatric preparation of codeine phosphate as well as powerful long-release opioids which can be administered per os , or percutaneously for transdermal fentanyl .
	manualset3
222481	7	420777	7	NULL	NULL	0	NULL	pediatric preparation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	NEW OPIOID ANALGESICS : Progress in pain reliet has recently been achieved with the introduction of new opioid analgesics such as tramadol and the pediatric preparation of codeine phosphate as well as powerful long-release opioids which can be administered per os , or percutaneously for transdermal fentanyl .
	manualset3
222482	8	420777	7	NULL	NULL	0	NULL	codeine phosphate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	NEW OPIOID ANALGESICS : Progress in pain reliet has recently been achieved with the introduction of new opioid analgesics such as tramadol and the pediatric preparation of codeine phosphate as well as powerful long-release opioids which can be administered per os , or percutaneously for transdermal fentanyl .
	manualset3
222483	9	420777	7	NULL	NULL	0	NULL	long-release opioids	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	NEW OPIOID ANALGESICS : Progress in pain reliet has recently been achieved with the introduction of new opioid analgesics such as tramadol and the pediatric preparation of codeine phosphate as well as powerful long-release opioids which can be administered per os , or percutaneously for transdermal fentanyl .
	manualset3
222484	10	420777	7	NULL	NULL	0	NULL	per os	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	NEW OPIOID ANALGESICS : Progress in pain reliet has recently been achieved with the introduction of new opioid analgesics such as tramadol and the pediatric preparation of codeine phosphate as well as powerful long-release opioids which can be administered per os , or percutaneously for transdermal fentanyl .
	manualset3
222485	11	420777	7	NULL	NULL	0	NULL	transdermal fentanyl 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	NEW OPIOID ANALGESICS : Progress in pain reliet has recently been achieved with the introduction of new opioid analgesics such as tramadol and the pediatric preparation of codeine phosphate as well as powerful long-release opioids which can be administered per os , or percutaneously for transdermal fentanyl .
	manualset3
222486	1	420778	7	NULL	NULL	0	NULL	Nonspecific inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonspecific inhibitors of cytochrome P-450 , such as ketoconazole , itraconazole , fluconazole and SKF 525 A , and most of the cytochrome P-450 IIIA specific substrates used in this study significantly inhibited FK 506 metabolism .
	manualset3
222487	2	420778	7	NULL	NULL	0	NULL	cytochrome P-450	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonspecific inhibitors of cytochrome P-450 , such as ketoconazole , itraconazole , fluconazole and SKF 525 A , and most of the cytochrome P-450 IIIA specific substrates used in this study significantly inhibited FK 506 metabolism .
	manualset3
222488	3	420778	7	NULL	NULL	0	NULL	ketoconazole 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonspecific inhibitors of cytochrome P-450 , such as ketoconazole , itraconazole , fluconazole and SKF 525 A , and most of the cytochrome P-450 IIIA specific substrates used in this study significantly inhibited FK 506 metabolism .
	manualset3
222489	4	420778	7	NULL	NULL	0	NULL	 itraconazole	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonspecific inhibitors of cytochrome P-450 , such as ketoconazole , itraconazole , fluconazole and SKF 525 A , and most of the cytochrome P-450 IIIA specific substrates used in this study significantly inhibited FK 506 metabolism .
	manualset3
222490	5	420778	7	NULL	NULL	0	NULL	 fluconazole	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonspecific inhibitors of cytochrome P-450 , such as ketoconazole , itraconazole , fluconazole and SKF 525 A , and most of the cytochrome P-450 IIIA specific substrates used in this study significantly inhibited FK 506 metabolism .
	manualset3
222491	6	420778	7	NULL	NULL	0	NULL	SKF 525 A	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonspecific inhibitors of cytochrome P-450 , such as ketoconazole , itraconazole , fluconazole and SKF 525 A , and most of the cytochrome P-450 IIIA specific substrates used in this study significantly inhibited FK 506 metabolism .
	manualset3
222492	7	420778	7	NULL	NULL	0	NULL	cytochrome P-450 IIIA specific substrates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonspecific inhibitors of cytochrome P-450 , such as ketoconazole , itraconazole , fluconazole and SKF 525 A , and most of the cytochrome P-450 IIIA specific substrates used in this study significantly inhibited FK 506 metabolism .
	manualset3
222493	8	420778	7	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonspecific inhibitors of cytochrome P-450 , such as ketoconazole , itraconazole , fluconazole and SKF 525 A , and most of the cytochrome P-450 IIIA specific substrates used in this study significantly inhibited FK 506 metabolism .
	manualset3
222494	9	420778	7	NULL	NULL	0	NULL	FK 506 metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonspecific inhibitors of cytochrome P-450 , such as ketoconazole , itraconazole , fluconazole and SKF 525 A , and most of the cytochrome P-450 IIIA specific substrates used in this study significantly inhibited FK 506 metabolism .
	manualset3
222495	1	420779	7	NULL	NULL	0	NULL	Patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in group B had significantly less visual analog scale values , longer absolute analgesia time , lesser swallowing difficulty and they were discharged earlier from the hospital when compared to patients in both groups D and G. Using both pre-operative dexamethasone IV injection with GNB has reduced postoperative pain and morbidity to a great extent than using either alone .
	manualset3
222496	2	420779	7	NULL	NULL	0	NULL	group B	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in group B had significantly less visual analog scale values , longer absolute analgesia time , lesser swallowing difficulty and they were discharged earlier from the hospital when compared to patients in both groups D and G. Using both pre-operative dexamethasone IV injection with GNB has reduced postoperative pain and morbidity to a great extent than using either alone .
	manualset3
222497	3	420779	7	NULL	NULL	0	NULL	 visual analog scale values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in group B had significantly less visual analog scale values , longer absolute analgesia time , lesser swallowing difficulty and they were discharged earlier from the hospital when compared to patients in both groups D and G. Using both pre-operative dexamethasone IV injection with GNB has reduced postoperative pain and morbidity to a great extent than using either alone .
	manualset3
222498	4	420779	7	NULL	NULL	0	NULL	longer absolute analgesia time	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in group B had significantly less visual analog scale values , longer absolute analgesia time , lesser swallowing difficulty and they were discharged earlier from the hospital when compared to patients in both groups D and G. Using both pre-operative dexamethasone IV injection with GNB has reduced postoperative pain and morbidity to a great extent than using either alone .
	manualset3
222499	5	420779	7	NULL	NULL	0	NULL	lesser swallowing difficulty	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in group B had significantly less visual analog scale values , longer absolute analgesia time , lesser swallowing difficulty and they were discharged earlier from the hospital when compared to patients in both groups D and G. Using both pre-operative dexamethasone IV injection with GNB has reduced postoperative pain and morbidity to a great extent than using either alone .
	manualset3
222500	6	420779	7	NULL	NULL	0	NULL	 hospital	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in group B had significantly less visual analog scale values , longer absolute analgesia time , lesser swallowing difficulty and they were discharged earlier from the hospital when compared to patients in both groups D and G. Using both pre-operative dexamethasone IV injection with GNB has reduced postoperative pain and morbidity to a great extent than using either alone .
	manualset3
222501	7	420779	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in group B had significantly less visual analog scale values , longer absolute analgesia time , lesser swallowing difficulty and they were discharged earlier from the hospital when compared to patients in both groups D and G. Using both pre-operative dexamethasone IV injection with GNB has reduced postoperative pain and morbidity to a great extent than using either alone .
	manualset3
222502	8	420779	7	NULL	NULL	0	NULL	 groups D	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in group B had significantly less visual analog scale values , longer absolute analgesia time , lesser swallowing difficulty and they were discharged earlier from the hospital when compared to patients in both groups D and G. Using both pre-operative dexamethasone IV injection with GNB has reduced postoperative pain and morbidity to a great extent than using either alone .
	manualset3
222503	9	420779	7	NULL	NULL	0	NULL	 groups G	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in group B had significantly less visual analog scale values , longer absolute analgesia time , lesser swallowing difficulty and they were discharged earlier from the hospital when compared to patients in both groups D and G. Using both pre-operative dexamethasone IV injection with GNB has reduced postoperative pain and morbidity to a great extent than using either alone .
	manualset3
222504	10	420779	7	NULL	NULL	0	NULL	pre-operative dexamethasone IV injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in group B had significantly less visual analog scale values , longer absolute analgesia time , lesser swallowing difficulty and they were discharged earlier from the hospital when compared to patients in both groups D and G. Using both pre-operative dexamethasone IV injection with GNB has reduced postoperative pain and morbidity to a great extent than using either alone .
	manualset3
222505	11	420779	7	NULL	NULL	0	NULL	GNB	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in group B had significantly less visual analog scale values , longer absolute analgesia time , lesser swallowing difficulty and they were discharged earlier from the hospital when compared to patients in both groups D and G. Using both pre-operative dexamethasone IV injection with GNB has reduced postoperative pain and morbidity to a great extent than using either alone .
	manualset3
222506	12	420779	7	NULL	NULL	0	NULL	postoperative pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in group B had significantly less visual analog scale values , longer absolute analgesia time , lesser swallowing difficulty and they were discharged earlier from the hospital when compared to patients in both groups D and G. Using both pre-operative dexamethasone IV injection with GNB has reduced postoperative pain and morbidity to a great extent than using either alone .
	manualset3
222507	13	420779	7	NULL	NULL	0	NULL	morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients in group B had significantly less visual analog scale values , longer absolute analgesia time , lesser swallowing difficulty and they were discharged earlier from the hospital when compared to patients in both groups D and G. Using both pre-operative dexamethasone IV injection with GNB has reduced postoperative pain and morbidity to a great extent than using either alone .
	manualset3
222508	1	420780	7	NULL	NULL	0	NULL	Wolbachia 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	While Wolbachia may influence the expression of heat shock proteins , we found that there was no effect on adult heat resistance when tested in terms of survival or virility following heat stress .
	manualset3
222509	2	420780	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While Wolbachia may influence the expression of heat shock proteins , we found that there was no effect on adult heat resistance when tested in terms of survival or virility following heat stress .
	manualset3
222510	3	420780	7	NULL	NULL	0	NULL	heat shock proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	While Wolbachia may influence the expression of heat shock proteins , we found that there was no effect on adult heat resistance when tested in terms of survival or virility following heat stress .
	manualset3
222511	4	420780	7	NULL	NULL	0	NULL	adult heat resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While Wolbachia may influence the expression of heat shock proteins , we found that there was no effect on adult heat resistance when tested in terms of survival or virility following heat stress .
	manualset3
222512	5	420780	7	NULL	NULL	0	NULL	survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	While Wolbachia may influence the expression of heat shock proteins , we found that there was no effect on adult heat resistance when tested in terms of survival or virility following heat stress .
	manualset3
222513	6	420780	7	NULL	NULL	0	NULL	 virility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While Wolbachia may influence the expression of heat shock proteins , we found that there was no effect on adult heat resistance when tested in terms of survival or virility following heat stress .
	manualset3
222514	7	420780	7	NULL	NULL	0	NULL	heat stress 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	While Wolbachia may influence the expression of heat shock proteins , we found that there was no effect on adult heat resistance when tested in terms of survival or virility following heat stress .
	manualset3
222515	1	420781	7	NULL	NULL	0	NULL	AIL	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	AIL should be included in the differential diagnosis of any maculopapular eruption of unknown etiology accompanied by lymphadenopathy .
	manualset3
222516	2	420781	7	NULL	NULL	0	NULL	differential diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	AIL should be included in the differential diagnosis of any maculopapular eruption of unknown etiology accompanied by lymphadenopathy .
	manualset3
222517	3	420781	7	NULL	NULL	0	NULL	maculopapular eruption	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	AIL should be included in the differential diagnosis of any maculopapular eruption of unknown etiology accompanied by lymphadenopathy .
	manualset3
222518	4	420781	7	NULL	NULL	0	NULL	etiology	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	AIL should be included in the differential diagnosis of any maculopapular eruption of unknown etiology accompanied by lymphadenopathy .
	manualset3
222519	5	420781	7	NULL	NULL	0	NULL	 lymphadenopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	AIL should be included in the differential diagnosis of any maculopapular eruption of unknown etiology accompanied by lymphadenopathy .
	manualset3
222520	1	420782	7	NULL	NULL	0	NULL	Neuroimaging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroimaging conducted 2 years after the first symptoms was typical for the advanced stage of Alzheimer 's disease ( AD ) , showing cortical brain atrophy , particularly within hippocampus , frontal and temporal cortex .
	manualset3
222521	2	420782	7	NULL	NULL	0	NULL	2 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroimaging conducted 2 years after the first symptoms was typical for the advanced stage of Alzheimer 's disease ( AD ) , showing cortical brain atrophy , particularly within hippocampus , frontal and temporal cortex .
	manualset3
222522	3	420782	7	NULL	NULL	0	NULL	first symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroimaging conducted 2 years after the first symptoms was typical for the advanced stage of Alzheimer 's disease ( AD ) , showing cortical brain atrophy , particularly within hippocampus , frontal and temporal cortex .
	manualset3
222523	4	420782	7	NULL	NULL	0	NULL	 advanced stage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroimaging conducted 2 years after the first symptoms was typical for the advanced stage of Alzheimer 's disease ( AD ) , showing cortical brain atrophy , particularly within hippocampus , frontal and temporal cortex .
	manualset3
222524	5	420782	7	NULL	NULL	0	NULL	Alzheimer 's disease ( AD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroimaging conducted 2 years after the first symptoms was typical for the advanced stage of Alzheimer 's disease ( AD ) , showing cortical brain atrophy , particularly within hippocampus , frontal and temporal cortex .
	manualset3
222525	6	420782	7	NULL	NULL	0	NULL	cortical brain atrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroimaging conducted 2 years after the first symptoms was typical for the advanced stage of Alzheimer 's disease ( AD ) , showing cortical brain atrophy , particularly within hippocampus , frontal and temporal cortex .
	manualset3
222526	7	420782	7	NULL	NULL	0	NULL	hippocampus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroimaging conducted 2 years after the first symptoms was typical for the advanced stage of Alzheimer 's disease ( AD ) , showing cortical brain atrophy , particularly within hippocampus , frontal and temporal cortex .
	manualset3
222527	8	420782	7	NULL	NULL	0	NULL	frontal cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroimaging conducted 2 years after the first symptoms was typical for the advanced stage of Alzheimer 's disease ( AD ) , showing cortical brain atrophy , particularly within hippocampus , frontal and temporal cortex .
	manualset3
222528	9	420782	7	NULL	NULL	0	NULL	temporal cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroimaging conducted 2 years after the first symptoms was typical for the advanced stage of Alzheimer 's disease ( AD ) , showing cortical brain atrophy , particularly within hippocampus , frontal and temporal cortex .
	manualset3
222529	1	420783	7	NULL	NULL	0	NULL	treatment group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	For the treatment group , rAd2p53 was injected into multiple areas of the lesion once a week for 6weeks avoiding deep ulcers points .
	manualset3
222530	2	420783	7	NULL	NULL	NULL	NULL	 rAd2p53	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For the treatment group , rAd2p53 was injected into multiple areas of the lesion once a week for 6weeks avoiding deep ulcers points .
	manualset3
222531	3	420783	7	NULL	NULL	0	NULL	multiple areas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For the treatment group , rAd2p53 was injected into multiple areas of the lesion once a week for 6weeks avoiding deep ulcers points .
	manualset3
222532	4	420783	7	NULL	NULL	0	NULL	lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For the treatment group , rAd2p53 was injected into multiple areas of the lesion once a week for 6weeks avoiding deep ulcers points .
	manualset3
222533	5	420783	7	NULL	NULL	0	NULL	week 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	For the treatment group , rAd2p53 was injected into multiple areas of the lesion once a week for 6weeks avoiding deep ulcers points .
	manualset3
222534	6	420783	7	NULL	NULL	0	NULL	6weeks 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	For the treatment group , rAd2p53 was injected into multiple areas of the lesion once a week for 6weeks avoiding deep ulcers points .
	manualset3
222535	7	420783	7	NULL	NULL	NULL	NULL	deep ulcers points	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For the treatment group , rAd2p53 was injected into multiple areas of the lesion once a week for 6weeks avoiding deep ulcers points .
	manualset3
222593	1	420784	7	NULL	NULL	0	NULL	 things	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among other things , serotonin enhances intestinal motility .
	manualset3
222594	2	420784	7	NULL	NULL	0	NULL	 serotonin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Among other things , serotonin enhances intestinal motility .
	manualset3
222595	3	420784	7	NULL	NULL	0	NULL	intestinal motility 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among other things , serotonin enhances intestinal motility .
	manualset3
222598	1	420785	7	NULL	NULL	0	NULL	reading frame 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The reading frame was composed of 65.5 % G + C with 82.3 % of the codons ending in G or C. There was no intergenic space between bkdA2 and bkdB .
	manualset3
222600	2	420785	7	NULL	NULL	0	NULL	65.5 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The reading frame was composed of 65.5 % G + C with 82.3 % of the codons ending in G or C. There was no intergenic space between bkdA2 and bkdB .
	manualset3
222602	3	420785	7	NULL	NULL	0	NULL	G + C 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The reading frame was composed of 65.5 % G + C with 82.3 % of the codons ending in G or C. There was no intergenic space between bkdA2 and bkdB .
	manualset3
222604	4	420785	7	NULL	NULL	0	NULL	82.3 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The reading frame was composed of 65.5 % G + C with 82.3 % of the codons ending in G or C. There was no intergenic space between bkdA2 and bkdB .
	manualset3
222606	5	420785	7	NULL	NULL	NULL	NULL	codons	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reading frame was composed of 65.5 % G + C with 82.3 % of the codons ending in G or C. There was no intergenic space between bkdA2 and bkdB .
	manualset3
222608	6	420785	7	NULL	NULL	0	NULL	G	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reading frame was composed of 65.5 % G + C with 82.3 % of the codons ending in G or C. There was no intergenic space between bkdA2 and bkdB .
	manualset3
222610	7	420785	7	NULL	NULL	0	NULL	C	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reading frame was composed of 65.5 % G + C with 82.3 % of the codons ending in G or C. There was no intergenic space between bkdA2 and bkdB .
	manualset3
222611	8	420785	7	NULL	NULL	0	NULL	intergenic space	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The reading frame was composed of 65.5 % G + C with 82.3 % of the codons ending in G or C. There was no intergenic space between bkdA2 and bkdB .
	manualset3
222612	9	420785	7	NULL	NULL	0	NULL	bkdA2 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The reading frame was composed of 65.5 % G + C with 82.3 % of the codons ending in G or C. There was no intergenic space between bkdA2 and bkdB .
	manualset3
222613	10	420785	7	NULL	NULL	0	NULL	bkdB	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The reading frame was composed of 65.5 % G + C with 82.3 % of the codons ending in G or C. There was no intergenic space between bkdA2 and bkdB .
	manualset3
222614	1	420786	7	NULL	NULL	0	NULL	availability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , availability of a large number of potent ligands of MCRs , especially those for the therapeutically important MC4R , has fueled ligand-based approaches , including automated pharmacophore query optimization and pharmacophore-based virtual screening .
	manualset3
222615	2	420786	7	NULL	NULL	0	NULL	 large number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , availability of a large number of potent ligands of MCRs , especially those for the therapeutically important MC4R , has fueled ligand-based approaches , including automated pharmacophore query optimization and pharmacophore-based virtual screening .
	manualset3
222617	3	420786	7	NULL	NULL	0	NULL	potent ligands	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , availability of a large number of potent ligands of MCRs , especially those for the therapeutically important MC4R , has fueled ligand-based approaches , including automated pharmacophore query optimization and pharmacophore-based virtual screening .
	manualset3
222618	4	420786	7	NULL	NULL	0	NULL	MCRs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , availability of a large number of potent ligands of MCRs , especially those for the therapeutically important MC4R , has fueled ligand-based approaches , including automated pharmacophore query optimization and pharmacophore-based virtual screening .
	manualset3
222620	5	420786	7	NULL	NULL	0	NULL	MC4R	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , availability of a large number of potent ligands of MCRs , especially those for the therapeutically important MC4R , has fueled ligand-based approaches , including automated pharmacophore query optimization and pharmacophore-based virtual screening .
	manualset3
222622	6	420786	7	NULL	NULL	0	NULL	ligand-based approaches	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , availability of a large number of potent ligands of MCRs , especially those for the therapeutically important MC4R , has fueled ligand-based approaches , including automated pharmacophore query optimization and pharmacophore-based virtual screening .
	manualset3
222624	7	420786	7	NULL	NULL	0	NULL	automated pharmacophore query optimization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , availability of a large number of potent ligands of MCRs , especially those for the therapeutically important MC4R , has fueled ligand-based approaches , including automated pharmacophore query optimization and pharmacophore-based virtual screening .
	manualset3
222626	8	420786	7	NULL	NULL	0	NULL	pharmacophore-based virtual screening	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , availability of a large number of potent ligands of MCRs , especially those for the therapeutically important MC4R , has fueled ligand-based approaches , including automated pharmacophore query optimization and pharmacophore-based virtual screening .
	manualset3
222629	1	420787	7	NULL	NULL	0	NULL	Factors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Factors that predict the benefit of lowering intraocular pressure in normal-tension glaucoma .
	manualset3
222630	2	420787	7	NULL	NULL	0	NULL	benefit 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Factors that predict the benefit of lowering intraocular pressure in normal-tension glaucoma .
	manualset3
222631	3	420787	7	NULL	NULL	0	NULL	intraocular pressure 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Factors that predict the benefit of lowering intraocular pressure in normal-tension glaucoma .
	manualset3
222632	4	420787	7	NULL	NULL	0	NULL	normal-tension glaucoma 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Factors that predict the benefit of lowering intraocular pressure in normal-tension glaucoma .
	manualset3
222636	1	420788	7	NULL	NULL	NULL	NULL	spectrum 	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When the spectrum of the probe in the cytoplasm is deconvoluted into the same components the mismatch is higher .
	manualset3
222637	2	420788	7	NULL	NULL	0	NULL	cytoplasm	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	When the spectrum of the probe in the cytoplasm is deconvoluted into the same components the mismatch is higher .
	manualset3
222638	3	420788	7	NULL	NULL	0	NULL	components 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	When the spectrum of the probe in the cytoplasm is deconvoluted into the same components the mismatch is higher .
	manualset3
222639	4	420788	7	NULL	NULL	0	NULL	mismatch	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When the spectrum of the probe in the cytoplasm is deconvoluted into the same components the mismatch is higher .
	manualset3
224179	5	420788	7	NULL	NULL	NULL	NULL	probe	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When the spectrum of the probe in the cytoplasm is deconvoluted into the same components the mismatch is higher .
	manualset3
222641	1	420789	7	NULL	NULL	0	NULL	Neurospora crassa glucogen phosphorylase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurospora crassa glucogen phosphorylase : interconversion and kinetic properties of the `` active '' form .
	manualset3
222643	2	420789	7	NULL	NULL	0	NULL	interconversion 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurospora crassa glucogen phosphorylase : interconversion and kinetic properties of the `` active '' form .
	manualset3
222645	3	420789	7	NULL	NULL	0	NULL	 kinetic properties	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurospora crassa glucogen phosphorylase : interconversion and kinetic properties of the `` active '' form .
	manualset3
222646	4	420789	7	NULL	NULL	0	NULL	 active '' form 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurospora crassa glucogen phosphorylase : interconversion and kinetic properties of the `` active '' form .
	manualset3
222647	1	420790	7	NULL	NULL	0	NULL	Administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Administration of a low dose of 4-methylpyrazole ( 4-MP ) that abolished acetaldehyde accumulation did not , however , remove the suppression produced by cyanamide .
	manualset3
222648	2	420790	7	NULL	NULL	0	NULL	low dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Administration of a low dose of 4-methylpyrazole ( 4-MP ) that abolished acetaldehyde accumulation did not , however , remove the suppression produced by cyanamide .
	manualset3
222649	3	420790	7	NULL	NULL	NULL	NULL	4-methylpyrazole ( 4-MP )	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Administration of a low dose of 4-methylpyrazole ( 4-MP ) that abolished acetaldehyde accumulation did not , however , remove the suppression produced by cyanamide .
	manualset3
222650	4	420790	7	NULL	NULL	0	NULL	acetaldehyde accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Administration of a low dose of 4-methylpyrazole ( 4-MP ) that abolished acetaldehyde accumulation did not , however , remove the suppression produced by cyanamide .
	manualset3
222651	5	420790	7	NULL	NULL	0	NULL	suppression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Administration of a low dose of 4-methylpyrazole ( 4-MP ) that abolished acetaldehyde accumulation did not , however , remove the suppression produced by cyanamide .
	manualset3
222652	6	420790	7	NULL	NULL	0	NULL	cyanamide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Administration of a low dose of 4-methylpyrazole ( 4-MP ) that abolished acetaldehyde accumulation did not , however , remove the suppression produced by cyanamide .
	manualset3
222653	1	420791	7	NULL	NULL	NULL	NULL	Fifty normal right knees	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fifty normal right knees in young adults ( group 1 ) and 50 knees from adults of various ages undergoing arthroscopic surgery for relatively simple intra-articular pathologies or diagnosis ( group 2 ) were included .
	manualset3
222654	2	420791	7	NULL	NULL	0	NULL	young adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Fifty normal right knees in young adults ( group 1 ) and 50 knees from adults of various ages undergoing arthroscopic surgery for relatively simple intra-articular pathologies or diagnosis ( group 2 ) were included .
	manualset3
222655	3	420791	7	NULL	NULL	0	NULL	group 1	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Fifty normal right knees in young adults ( group 1 ) and 50 knees from adults of various ages undergoing arthroscopic surgery for relatively simple intra-articular pathologies or diagnosis ( group 2 ) were included .
	manualset3
222656	4	420791	7	NULL	NULL	0	NULL	50 knees	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Fifty normal right knees in young adults ( group 1 ) and 50 knees from adults of various ages undergoing arthroscopic surgery for relatively simple intra-articular pathologies or diagnosis ( group 2 ) were included .
	manualset3
222659	5	420791	7	NULL	NULL	0	NULL	adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Fifty normal right knees in young adults ( group 1 ) and 50 knees from adults of various ages undergoing arthroscopic surgery for relatively simple intra-articular pathologies or diagnosis ( group 2 ) were included .
	manualset3
222661	6	420791	7	NULL	NULL	0	NULL	ages	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Fifty normal right knees in young adults ( group 1 ) and 50 knees from adults of various ages undergoing arthroscopic surgery for relatively simple intra-articular pathologies or diagnosis ( group 2 ) were included .
	manualset3
222663	7	420791	7	NULL	NULL	0	NULL	arthroscopic surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Fifty normal right knees in young adults ( group 1 ) and 50 knees from adults of various ages undergoing arthroscopic surgery for relatively simple intra-articular pathologies or diagnosis ( group 2 ) were included .
	manualset3
222666	8	420791	7	NULL	NULL	0	NULL	 intra-articular pathologies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Fifty normal right knees in young adults ( group 1 ) and 50 knees from adults of various ages undergoing arthroscopic surgery for relatively simple intra-articular pathologies or diagnosis ( group 2 ) were included .
	manualset3
222667	9	420791	7	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Fifty normal right knees in young adults ( group 1 ) and 50 knees from adults of various ages undergoing arthroscopic surgery for relatively simple intra-articular pathologies or diagnosis ( group 2 ) were included .
	manualset3
222668	10	420791	7	NULL	NULL	0	NULL	group 2	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Fifty normal right knees in young adults ( group 1 ) and 50 knees from adults of various ages undergoing arthroscopic surgery for relatively simple intra-articular pathologies or diagnosis ( group 2 ) were included .
	manualset3
222672	1	420792	7	NULL	NULL	0	NULL	underlying reasons	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among other underlying reasons , poorer counties tend to have high-density populations and more children and other higher-risk people per household , resulting in more interactions and both increased transmission of influenza and greater risk for worse influenza outcomes .
	manualset3
222675	2	420792	7	NULL	NULL	NULL	NULL	poorer counties	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Among other underlying reasons , poorer counties tend to have high-density populations and more children and other higher-risk people per household , resulting in more interactions and both increased transmission of influenza and greater risk for worse influenza outcomes .
	manualset3
222676	3	420792	7	NULL	NULL	0	NULL	high-density populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among other underlying reasons , poorer counties tend to have high-density populations and more children and other higher-risk people per household , resulting in more interactions and both increased transmission of influenza and greater risk for worse influenza outcomes .
	manualset3
222677	4	420792	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among other underlying reasons , poorer counties tend to have high-density populations and more children and other higher-risk people per household , resulting in more interactions and both increased transmission of influenza and greater risk for worse influenza outcomes .
	manualset3
222678	5	420792	7	NULL	NULL	0	NULL	higher-risk people per household	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among other underlying reasons , poorer counties tend to have high-density populations and more children and other higher-risk people per household , resulting in more interactions and both increased transmission of influenza and greater risk for worse influenza outcomes .
	manualset3
222679	6	420792	7	NULL	NULL	0	NULL	 interactions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among other underlying reasons , poorer counties tend to have high-density populations and more children and other higher-risk people per household , resulting in more interactions and both increased transmission of influenza and greater risk for worse influenza outcomes .
	manualset3
222680	7	420792	7	NULL	NULL	0	NULL	transmission	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among other underlying reasons , poorer counties tend to have high-density populations and more children and other higher-risk people per household , resulting in more interactions and both increased transmission of influenza and greater risk for worse influenza outcomes .
	manualset3
222681	8	420792	7	NULL	NULL	0	NULL	influenza	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among other underlying reasons , poorer counties tend to have high-density populations and more children and other higher-risk people per household , resulting in more interactions and both increased transmission of influenza and greater risk for worse influenza outcomes .
	manualset3
222682	9	420792	7	NULL	NULL	0	NULL	greater risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among other underlying reasons , poorer counties tend to have high-density populations and more children and other higher-risk people per household , resulting in more interactions and both increased transmission of influenza and greater risk for worse influenza outcomes .
	manualset3
222683	10	420792	7	NULL	NULL	0	NULL	worse influenza outcomes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among other underlying reasons , poorer counties tend to have high-density populations and more children and other higher-risk people per household , resulting in more interactions and both increased transmission of influenza and greater risk for worse influenza outcomes .
	manualset3
222686	1	420793	7	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of indoor plantings as allergen sources was assessed by direct sampling of interior air .
	manualset3
222687	2	420793	7	NULL	NULL	0	NULL	indoor plantings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of indoor plantings as allergen sources was assessed by direct sampling of interior air .
	manualset3
222688	3	420793	7	NULL	NULL	0	NULL	 allergen sources	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of indoor plantings as allergen sources was assessed by direct sampling of interior air .
	manualset3
222689	4	420793	7	NULL	NULL	0	NULL	direct sampling 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of indoor plantings as allergen sources was assessed by direct sampling of interior air .
	manualset3
222690	5	420793	7	NULL	NULL	0	NULL	interior air 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of indoor plantings as allergen sources was assessed by direct sampling of interior air .
	manualset3
222707	1	420794	7	NULL	NULL	0	NULL	Revertant frequencies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Revertant frequencies observed in parallel in the strains TA100 and TA2638 indicate a pronounced mutagenicity of the lesions induced .
	manualset3
222708	2	420794	7	NULL	NULL	0	NULL	strains TA100	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Revertant frequencies observed in parallel in the strains TA100 and TA2638 indicate a pronounced mutagenicity of the lesions induced .
	manualset3
222709	3	420794	7	NULL	NULL	0	NULL	TA2638 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Revertant frequencies observed in parallel in the strains TA100 and TA2638 indicate a pronounced mutagenicity of the lesions induced .
	manualset3
222711	4	420794	7	NULL	NULL	0	NULL	mutagenicity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Revertant frequencies observed in parallel in the strains TA100 and TA2638 indicate a pronounced mutagenicity of the lesions induced .
	manualset3
222715	5	420794	7	NULL	NULL	0	NULL	lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Revertant frequencies observed in parallel in the strains TA100 and TA2638 indicate a pronounced mutagenicity of the lesions induced .
	manualset3
222721	1	420795	7	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , cell-cycle arrest of BGC-823 human gastric carcinoma cells caused by oroxylin A has been investigated .
	manualset3
222722	2	420795	7	NULL	NULL	0	NULL	cell-cycle arrest	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , cell-cycle arrest of BGC-823 human gastric carcinoma cells caused by oroxylin A has been investigated .
	manualset3
222723	3	420795	7	NULL	NULL	0	NULL	BGC-823 human gastric carcinoma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , cell-cycle arrest of BGC-823 human gastric carcinoma cells caused by oroxylin A has been investigated .
	manualset3
222724	4	420795	7	NULL	NULL	0	NULL	 oroxylin A	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , cell-cycle arrest of BGC-823 human gastric carcinoma cells caused by oroxylin A has been investigated .
	manualset3
222725	1	420796	7	NULL	NULL	0	NULL	ICS	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	When ICS are administered at high doses , secondary adrenal insufficiency due to the excessive exogenous corticosteroid certainly may become manifest .
	manualset3
222726	2	420796	7	NULL	NULL	0	NULL	 high doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When ICS are administered at high doses , secondary adrenal insufficiency due to the excessive exogenous corticosteroid certainly may become manifest .
	manualset3
222727	3	420796	7	NULL	NULL	0	NULL	secondary adrenal insufficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	When ICS are administered at high doses , secondary adrenal insufficiency due to the excessive exogenous corticosteroid certainly may become manifest .
	manualset3
222728	4	420796	7	NULL	NULL	0	NULL	excessive exogenous corticosteroid	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	When ICS are administered at high doses , secondary adrenal insufficiency due to the excessive exogenous corticosteroid certainly may become manifest .
	manualset3
222729	1	420797	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study demonstrates that graded meshes , for potential application in interfacial tissue engineering , can be fabricated by co-electrospinning .
	manualset3
222730	2	420797	7	NULL	NULL	0	NULL	graded meshes	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The study demonstrates that graded meshes , for potential application in interfacial tissue engineering , can be fabricated by co-electrospinning .
	manualset3
222731	3	420797	7	NULL	NULL	0	NULL	potential application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The study demonstrates that graded meshes , for potential application in interfacial tissue engineering , can be fabricated by co-electrospinning .
	manualset3
222732	4	420797	7	NULL	NULL	0	NULL	interfacial tissue engineering	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The study demonstrates that graded meshes , for potential application in interfacial tissue engineering , can be fabricated by co-electrospinning .
	manualset3
222733	5	420797	7	NULL	NULL	0	NULL	co-electrospinning	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study demonstrates that graded meshes , for potential application in interfacial tissue engineering , can be fabricated by co-electrospinning .
	manualset3
222734	1	420798	7	NULL	NULL	0	NULL	Symptomatic relief	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Symptomatic relief was achieved in five patients with rapidly progressive neurological disease who died within 27 months .
	manualset3
222735	2	420798	7	NULL	NULL	0	NULL	five patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Symptomatic relief was achieved in five patients with rapidly progressive neurological disease who died within 27 months .
	manualset3
222791	3	420798	7	NULL	NULL	0	NULL	progressive neurological disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Symptomatic relief was achieved in five patients with rapidly progressive neurological disease who died within 27 months .
	manualset3
222792	4	420798	7	NULL	NULL	0	NULL	27 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Symptomatic relief was achieved in five patients with rapidly progressive neurological disease who died within 27 months .
	manualset3
222793	1	420799	7	NULL	NULL	0	NULL	Case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Case of septicemia caused by postabortal Clostridium perfringens infection with anuria treated by exchange transfusion and tifomycin ) .
	manualset3
222795	2	420799	7	NULL	NULL	0	NULL	septicemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Case of septicemia caused by postabortal Clostridium perfringens infection with anuria treated by exchange transfusion and tifomycin ) .
	manualset3
222796	3	420799	7	NULL	NULL	0	NULL	postabortal Clostridium perfringens infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Case of septicemia caused by postabortal Clostridium perfringens infection with anuria treated by exchange transfusion and tifomycin ) .
	manualset3
222797	4	420799	7	NULL	NULL	0	NULL	anuria	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Case of septicemia caused by postabortal Clostridium perfringens infection with anuria treated by exchange transfusion and tifomycin ) .
	manualset3
222798	5	420799	7	NULL	NULL	0	NULL	exchange transfusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Case of septicemia caused by postabortal Clostridium perfringens infection with anuria treated by exchange transfusion and tifomycin ) .
	manualset3
222800	6	420799	7	NULL	NULL	0	NULL	tifomycin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Case of septicemia caused by postabortal Clostridium perfringens infection with anuria treated by exchange transfusion and tifomycin ) .
	manualset3
222831	1	420800	7	NULL	NULL	0	NULL	 premenopausal women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among premenopausal women , race/ethnicity , depression , and lower relationship happiness were also associated with combined arousal/lubrication problems .
	manualset3
222832	2	420800	7	NULL	NULL	0	NULL	 race/ethnicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among premenopausal women , race/ethnicity , depression , and lower relationship happiness were also associated with combined arousal/lubrication problems .
	manualset3
222833	3	420800	7	NULL	NULL	0	NULL	depression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among premenopausal women , race/ethnicity , depression , and lower relationship happiness were also associated with combined arousal/lubrication problems .
	manualset3
222834	4	420800	7	NULL	NULL	0	NULL	 lower relationship happiness 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among premenopausal women , race/ethnicity , depression , and lower relationship happiness were also associated with combined arousal/lubrication problems .
	manualset3
222835	5	420800	7	NULL	NULL	0	NULL	combined arousal/lubrication problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among premenopausal women , race/ethnicity , depression , and lower relationship happiness were also associated with combined arousal/lubrication problems .
	manualset3
222836	1	420801	7	NULL	NULL	0	NULL	theory	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Any theory that accounts for the concrete-noun effect must also be able to account for the effect of referent familiarity , and our results are discussed within this context .
	manualset3
222837	2	420801	7	NULL	NULL	0	NULL	concrete-noun effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Any theory that accounts for the concrete-noun effect must also be able to account for the effect of referent familiarity , and our results are discussed within this context .
	manualset3
222838	3	420801	7	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Any theory that accounts for the concrete-noun effect must also be able to account for the effect of referent familiarity , and our results are discussed within this context .
	manualset3
222839	4	420801	7	NULL	NULL	0	NULL	 referent familiarity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Any theory that accounts for the concrete-noun effect must also be able to account for the effect of referent familiarity , and our results are discussed within this context .
	manualset3
222840	5	420801	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Any theory that accounts for the concrete-noun effect must also be able to account for the effect of referent familiarity , and our results are discussed within this context .
	manualset3
222841	6	420801	7	NULL	NULL	0	NULL	context	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Any theory that accounts for the concrete-noun effect must also be able to account for the effect of referent familiarity , and our results are discussed within this context .
	manualset3
222842	1	420802	7	NULL	NULL	0	NULL	major source 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Because the major source of heat to the airways is provided by its microcirculation , inhaled furosemide may be acting as a topical vasodilator serving to enhance heat availability and thus reducing the effective thermal burden of hyperpnea .
	manualset3
222843	2	420802	7	NULL	NULL	0	NULL	heat 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Because the major source of heat to the airways is provided by its microcirculation , inhaled furosemide may be acting as a topical vasodilator serving to enhance heat availability and thus reducing the effective thermal burden of hyperpnea .
	manualset3
222844	3	420802	7	NULL	NULL	0	NULL	airways	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Because the major source of heat to the airways is provided by its microcirculation , inhaled furosemide may be acting as a topical vasodilator serving to enhance heat availability and thus reducing the effective thermal burden of hyperpnea .
	manualset3
222845	4	420802	7	NULL	NULL	0	NULL	microcirculation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Because the major source of heat to the airways is provided by its microcirculation , inhaled furosemide may be acting as a topical vasodilator serving to enhance heat availability and thus reducing the effective thermal burden of hyperpnea .
	manualset3
222846	5	420802	7	NULL	NULL	0	NULL	inhaled furosemide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Because the major source of heat to the airways is provided by its microcirculation , inhaled furosemide may be acting as a topical vasodilator serving to enhance heat availability and thus reducing the effective thermal burden of hyperpnea .
	manualset3
222847	6	420802	7	NULL	NULL	0	NULL	topical vasodilator	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Because the major source of heat to the airways is provided by its microcirculation , inhaled furosemide may be acting as a topical vasodilator serving to enhance heat availability and thus reducing the effective thermal burden of hyperpnea .
	manualset3
222848	7	420802	7	NULL	NULL	0	NULL	heat availability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Because the major source of heat to the airways is provided by its microcirculation , inhaled furosemide may be acting as a topical vasodilator serving to enhance heat availability and thus reducing the effective thermal burden of hyperpnea .
	manualset3
222849	8	420802	7	NULL	NULL	NULL	NULL	thermal burden 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the major source of heat to the airways is provided by its microcirculation , inhaled furosemide may be acting as a topical vasodilator serving to enhance heat availability and thus reducing the effective thermal burden of hyperpnea .
	manualset3
222850	9	420802	7	NULL	NULL	0	NULL	hyperpnea	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Because the major source of heat to the airways is provided by its microcirculation , inhaled furosemide may be acting as a topical vasodilator serving to enhance heat availability and thus reducing the effective thermal burden of hyperpnea .
	manualset3
222851	1	420803	7	NULL	NULL	0	NULL	Areas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Areas of high attenuation ( visually as opaque as bony structures ) in an abnormality on CT scans can be an important clue to the correct diagnosis .
	manualset3
222852	2	420803	7	NULL	NULL	0	NULL	high attenuation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Areas of high attenuation ( visually as opaque as bony structures ) in an abnormality on CT scans can be an important clue to the correct diagnosis .
	manualset3
222853	3	420803	7	NULL	NULL	0	NULL	bony structures	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Areas of high attenuation ( visually as opaque as bony structures ) in an abnormality on CT scans can be an important clue to the correct diagnosis .
	manualset3
222854	4	420803	7	NULL	NULL	0	NULL	abnormality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Areas of high attenuation ( visually as opaque as bony structures ) in an abnormality on CT scans can be an important clue to the correct diagnosis .
	manualset3
222855	5	420803	7	NULL	NULL	0	NULL	CT scans	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Areas of high attenuation ( visually as opaque as bony structures ) in an abnormality on CT scans can be an important clue to the correct diagnosis .
	manualset3
222856	6	420803	7	NULL	NULL	0	NULL	important clue	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Areas of high attenuation ( visually as opaque as bony structures ) in an abnormality on CT scans can be an important clue to the correct diagnosis .
	manualset3
222857	7	420803	7	NULL	NULL	0	NULL	correct diagnosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Areas of high attenuation ( visually as opaque as bony structures ) in an abnormality on CT scans can be an important clue to the correct diagnosis .
	manualset3
222858	1	420804	7	NULL	NULL	0	NULL	finding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important finding was the occurrence of cases caused by serotype O8 Yersinia enterocolitica in our country .
	manualset3
222859	2	420804	7	NULL	NULL	0	NULL	cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important finding was the occurrence of cases caused by serotype O8 Yersinia enterocolitica in our country .
	manualset3
222860	3	420804	7	NULL	NULL	0	NULL	 serotype O8 Yersinia enterocolitica	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important finding was the occurrence of cases caused by serotype O8 Yersinia enterocolitica in our country .
	manualset3
222861	4	420804	7	NULL	NULL	0	NULL	country	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important finding was the occurrence of cases caused by serotype O8 Yersinia enterocolitica in our country .
	manualset3
222862	5	420804	7	NULL	NULL	0	NULL	 occurrence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important finding was the occurrence of cases caused by serotype O8 Yersinia enterocolitica in our country .
	manualset3
222863	1	420805	7	NULL	NULL	0	NULL	Progressive supranuclear palsy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Progressive supranuclear palsy with wall-eyed bilateral internuclear ophthalmoplegia syndrome .
	manualset3
222864	2	420805	7	NULL	NULL	0	NULL	wall-eyed bilateral internuclear ophthalmoplegia syndrome 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Progressive supranuclear palsy with wall-eyed bilateral internuclear ophthalmoplegia syndrome .
	manualset3
222865	1	420806	7	NULL	NULL	0	NULL	rhesus monkey	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A rhesus monkey with a naturally acquired STLV-III infection developed immunosuppression and a lymphoproliferative syndrome characterized by progressive lymphadenopathy and widespread visceral mononuclear cell infiltration .
	manualset3
222866	2	420806	7	NULL	NULL	0	NULL	naturally acquired STLV-III infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A rhesus monkey with a naturally acquired STLV-III infection developed immunosuppression and a lymphoproliferative syndrome characterized by progressive lymphadenopathy and widespread visceral mononuclear cell infiltration .
	manualset3
222867	3	420806	7	NULL	NULL	0	NULL	 immunosuppression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A rhesus monkey with a naturally acquired STLV-III infection developed immunosuppression and a lymphoproliferative syndrome characterized by progressive lymphadenopathy and widespread visceral mononuclear cell infiltration .
	manualset3
222868	4	420806	7	NULL	NULL	0	NULL	lymphoproliferative syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A rhesus monkey with a naturally acquired STLV-III infection developed immunosuppression and a lymphoproliferative syndrome characterized by progressive lymphadenopathy and widespread visceral mononuclear cell infiltration .
	manualset3
222869	5	420806	7	NULL	NULL	0	NULL	progressive lymphadenopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A rhesus monkey with a naturally acquired STLV-III infection developed immunosuppression and a lymphoproliferative syndrome characterized by progressive lymphadenopathy and widespread visceral mononuclear cell infiltration .
	manualset3
222870	6	420806	7	NULL	NULL	0	NULL	visceral mononuclear cell infiltration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A rhesus monkey with a naturally acquired STLV-III infection developed immunosuppression and a lymphoproliferative syndrome characterized by progressive lymphadenopathy and widespread visceral mononuclear cell infiltration .
	manualset3
222871	1	420807	7	NULL	NULL	0	NULL	basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of initial rate studies , the kcat and Km values for TPAA were estimated to be 20-fold lower and 80-fold higher than the corresponding values for 2 , 4-D .
	manualset3
222872	2	420807	7	NULL	NULL	0	NULL	initial rate studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of initial rate studies , the kcat and Km values for TPAA were estimated to be 20-fold lower and 80-fold higher than the corresponding values for 2 , 4-D .
	manualset3
222873	3	420807	7	NULL	NULL	0	NULL	kcat values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of initial rate studies , the kcat and Km values for TPAA were estimated to be 20-fold lower and 80-fold higher than the corresponding values for 2 , 4-D .
	manualset3
222874	4	420807	7	NULL	NULL	0	NULL	Km values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of initial rate studies , the kcat and Km values for TPAA were estimated to be 20-fold lower and 80-fold higher than the corresponding values for 2 , 4-D .
	manualset3
222875	5	420807	7	NULL	NULL	0	NULL	TPAA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of initial rate studies , the kcat and Km values for TPAA were estimated to be 20-fold lower and 80-fold higher than the corresponding values for 2 , 4-D .
	manualset3
222876	6	420807	7	NULL	NULL	0	NULL	 20-fold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of initial rate studies , the kcat and Km values for TPAA were estimated to be 20-fold lower and 80-fold higher than the corresponding values for 2 , 4-D .
	manualset3
222877	7	420807	7	NULL	NULL	0	NULL	80-fold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of initial rate studies , the kcat and Km values for TPAA were estimated to be 20-fold lower and 80-fold higher than the corresponding values for 2 , 4-D .
	manualset3
222878	8	420807	7	NULL	NULL	0	NULL	corresponding values 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of initial rate studies , the kcat and Km values for TPAA were estimated to be 20-fold lower and 80-fold higher than the corresponding values for 2 , 4-D .
	manualset3
222879	9	420807	7	NULL	NULL	0	NULL	2 , 4-D	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of initial rate studies , the kcat and Km values for TPAA were estimated to be 20-fold lower and 80-fold higher than the corresponding values for 2 , 4-D .
	manualset3
222880	1	420808	7	NULL	NULL	0	NULL	Dermatopathia pigmentosa reticularis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Dermatopathia pigmentosa reticularis ) .
	manualset3
222881	1	420809	7	NULL	NULL	0	NULL	 generalized linear models ( GLM )	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We applied generalized linear models ( GLM ) for quantifying the estimated effects of DTR on mortality after adjusting for mean temperature , dew point temperature , day of the week , and seasonal and long-term trends .
	manualset3
222882	2	420809	7	NULL	NULL	0	NULL	estimated effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We applied generalized linear models ( GLM ) for quantifying the estimated effects of DTR on mortality after adjusting for mean temperature , dew point temperature , day of the week , and seasonal and long-term trends .
	manualset3
222883	3	420809	7	NULL	NULL	0	NULL	DTR	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We applied generalized linear models ( GLM ) for quantifying the estimated effects of DTR on mortality after adjusting for mean temperature , dew point temperature , day of the week , and seasonal and long-term trends .
	manualset3
222884	4	420809	7	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We applied generalized linear models ( GLM ) for quantifying the estimated effects of DTR on mortality after adjusting for mean temperature , dew point temperature , day of the week , and seasonal and long-term trends .
	manualset3
222885	5	420809	7	NULL	NULL	0	NULL	 mean temperature	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We applied generalized linear models ( GLM ) for quantifying the estimated effects of DTR on mortality after adjusting for mean temperature , dew point temperature , day of the week , and seasonal and long-term trends .
	manualset3
222886	6	420809	7	NULL	NULL	0	NULL	dew point temperature	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We applied generalized linear models ( GLM ) for quantifying the estimated effects of DTR on mortality after adjusting for mean temperature , dew point temperature , day of the week , and seasonal and long-term trends .
	manualset3
222887	7	420809	7	NULL	NULL	0	NULL	day	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	We applied generalized linear models ( GLM ) for quantifying the estimated effects of DTR on mortality after adjusting for mean temperature , dew point temperature , day of the week , and seasonal and long-term trends .
	manualset3
222888	8	420809	7	NULL	NULL	0	NULL	 week	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	We applied generalized linear models ( GLM ) for quantifying the estimated effects of DTR on mortality after adjusting for mean temperature , dew point temperature , day of the week , and seasonal and long-term trends .
	manualset3
222889	9	420809	7	NULL	NULL	0	NULL	seasonal trends	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We applied generalized linear models ( GLM ) for quantifying the estimated effects of DTR on mortality after adjusting for mean temperature , dew point temperature , day of the week , and seasonal and long-term trends .
	manualset3
222890	10	420809	7	NULL	NULL	0	NULL	long-term trends	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We applied generalized linear models ( GLM ) for quantifying the estimated effects of DTR on mortality after adjusting for mean temperature , dew point temperature , day of the week , and seasonal and long-term trends .
	manualset3
222891	1	420810	7	NULL	NULL	0	NULL	way	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Until now , there is no way to successful prevention and treatment of this problem .
	manualset3
222892	2	420810	7	NULL	NULL	0	NULL	 prevention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Until now , there is no way to successful prevention and treatment of this problem .
	manualset3
222893	3	420810	7	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Until now , there is no way to successful prevention and treatment of this problem .
	manualset3
222894	4	420810	7	NULL	NULL	0	NULL	problem	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Until now , there is no way to successful prevention and treatment of this problem .
	manualset3
222895	1	420811	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results confirm those of the standardization team in respect of granulated and cube sugar .
	manualset3
222896	2	420811	7	NULL	NULL	0	NULL	standardization team	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results confirm those of the standardization team in respect of granulated and cube sugar .
	manualset3
222897	3	420811	7	NULL	NULL	0	NULL	granulated and cube sugar	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results confirm those of the standardization team in respect of granulated and cube sugar .
	manualset3
222898	1	420812	7	NULL	NULL	0	NULL	Acyl-RAC	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Acyl-RAC should therefore find general applicability in studies of both global and individual protein S-acylation in mammalian cells .
	manualset3
222899	2	420812	7	NULL	NULL	0	NULL	general applicability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Acyl-RAC should therefore find general applicability in studies of both global and individual protein S-acylation in mammalian cells .
	manualset3
222900	3	420812	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Acyl-RAC should therefore find general applicability in studies of both global and individual protein S-acylation in mammalian cells .
	manualset3
222901	4	420812	7	NULL	NULL	0	NULL	global protein S-acylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acyl-RAC should therefore find general applicability in studies of both global and individual protein S-acylation in mammalian cells .
	manualset3
222902	5	420812	7	NULL	NULL	0	NULL	individual protein S-acylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acyl-RAC should therefore find general applicability in studies of both global and individual protein S-acylation in mammalian cells .
	manualset3
222903	6	420812	7	NULL	NULL	0	NULL	mammalian cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Acyl-RAC should therefore find general applicability in studies of both global and individual protein S-acylation in mammalian cells .
	manualset3
222904	1	420813	7	NULL	NULL	0	NULL	Tumor regression	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor regression was observed following either estrogen ablation alone or estrogen ablation in combination with tamoxifen .
	manualset3
222905	2	420813	7	NULL	NULL	NULL	NULL	estrogen ablation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Tumor regression was observed following either estrogen ablation alone or estrogen ablation in combination with tamoxifen .
	manualset3
222906	3	420813	7	NULL	NULL	0	NULL	estrogen ablation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor regression was observed following either estrogen ablation alone or estrogen ablation in combination with tamoxifen .
	manualset3
222907	4	420813	7	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor regression was observed following either estrogen ablation alone or estrogen ablation in combination with tamoxifen .
	manualset3
222908	5	420813	7	NULL	NULL	0	NULL	tamoxifen	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Tumor regression was observed following either estrogen ablation alone or estrogen ablation in combination with tamoxifen .
	manualset3
222909	1	420814	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This study illustrates that the Dutch version of the SDQ , similar to the English and German versions , has equal validity as the Dutch ASEBA for screening children .
	manualset3
222910	2	420814	7	NULL	NULL	0	NULL	Dutch version 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This study illustrates that the Dutch version of the SDQ , similar to the English and German versions , has equal validity as the Dutch ASEBA for screening children .
	manualset3
222911	3	420814	7	NULL	NULL	0	NULL	SDQ	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This study illustrates that the Dutch version of the SDQ , similar to the English and German versions , has equal validity as the Dutch ASEBA for screening children .
	manualset3
222912	4	420814	7	NULL	NULL	0	NULL	English versions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This study illustrates that the Dutch version of the SDQ , similar to the English and German versions , has equal validity as the Dutch ASEBA for screening children .
	manualset3
222913	5	420814	7	NULL	NULL	0	NULL	German versions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This study illustrates that the Dutch version of the SDQ , similar to the English and German versions , has equal validity as the Dutch ASEBA for screening children .
	manualset3
222914	6	420814	7	NULL	NULL	0	NULL	equal validity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This study illustrates that the Dutch version of the SDQ , similar to the English and German versions , has equal validity as the Dutch ASEBA for screening children .
	manualset3
222915	7	420814	7	NULL	NULL	0	NULL	Dutch ASEBA	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This study illustrates that the Dutch version of the SDQ , similar to the English and German versions , has equal validity as the Dutch ASEBA for screening children .
	manualset3
222916	8	420814	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This study illustrates that the Dutch version of the SDQ , similar to the English and German versions , has equal validity as the Dutch ASEBA for screening children .
	manualset3
222917	1	420815	7	NULL	NULL	0	NULL	diagnostic tests	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Among routinely used diagnostic tests , none were consistently indicative of WND , with the exception of the 24-h urine-Cu test , which is always outside the normal range .
	manualset3
222918	2	420815	7	NULL	NULL	0	NULL	WND	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Among routinely used diagnostic tests , none were consistently indicative of WND , with the exception of the 24-h urine-Cu test , which is always outside the normal range .
	manualset3
222919	3	420815	7	NULL	NULL	0	NULL	exception	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among routinely used diagnostic tests , none were consistently indicative of WND , with the exception of the 24-h urine-Cu test , which is always outside the normal range .
	manualset3
222920	4	420815	7	NULL	NULL	0	NULL	 24-h urine-Cu test	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Among routinely used diagnostic tests , none were consistently indicative of WND , with the exception of the 24-h urine-Cu test , which is always outside the normal range .
	manualset3
222921	5	420815	7	NULL	NULL	0	NULL	normal range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among routinely used diagnostic tests , none were consistently indicative of WND , with the exception of the 24-h urine-Cu test , which is always outside the normal range .
	manualset3
222922	1	420816	7	NULL	NULL	0	NULL	mineral salts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to mineral salts , xylem sap contains hormones , organic nutrients and proteins .
	manualset3
222923	2	420816	7	NULL	NULL	0	NULL	xylem sap	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to mineral salts , xylem sap contains hormones , organic nutrients and proteins .
	manualset3
222924	3	420816	7	NULL	NULL	0	NULL	hormones	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to mineral salts , xylem sap contains hormones , organic nutrients and proteins .
	manualset3
222925	4	420816	7	NULL	NULL	0	NULL	organic nutrients	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to mineral salts , xylem sap contains hormones , organic nutrients and proteins .
	manualset3
222926	5	420816	7	NULL	NULL	0	NULL	 proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to mineral salts , xylem sap contains hormones , organic nutrients and proteins .
	manualset3
222927	1	420817	7	NULL	NULL	0	NULL	patterns	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We examined patterns of perfectionism among college students and their biological parents in a sample of 188 undergraduates from intact families .
	manualset3
222928	2	420817	7	NULL	NULL	0	NULL	perfectionism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We examined patterns of perfectionism among college students and their biological parents in a sample of 188 undergraduates from intact families .
	manualset3
222929	3	420817	7	NULL	NULL	0	NULL	college students	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We examined patterns of perfectionism among college students and their biological parents in a sample of 188 undergraduates from intact families .
	manualset3
222930	4	420817	7	NULL	NULL	0	NULL	biological parents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We examined patterns of perfectionism among college students and their biological parents in a sample of 188 undergraduates from intact families .
	manualset3
222931	5	420817	7	NULL	NULL	0	NULL	 sample	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We examined patterns of perfectionism among college students and their biological parents in a sample of 188 undergraduates from intact families .
	manualset3
222932	6	420817	7	NULL	NULL	0	NULL	188 undergraduates	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We examined patterns of perfectionism among college students and their biological parents in a sample of 188 undergraduates from intact families .
	manualset3
222933	7	420817	7	NULL	NULL	0	NULL	intact families	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	We examined patterns of perfectionism among college students and their biological parents in a sample of 188 undergraduates from intact families .
	manualset3
222934	1	420818	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , LOWE suppressed compound 48/80-induced systemic allergic reaction and serum histamine release in mice and IgE-mediated local allergic reactions .
	manualset3
222935	2	420818	7	NULL	NULL	0	NULL	LOWE	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , LOWE suppressed compound 48/80-induced systemic allergic reaction and serum histamine release in mice and IgE-mediated local allergic reactions .
	manualset3
222936	3	420818	7	NULL	NULL	NULL	NULL	compound 48/80-induced systemic allergic reaction	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , LOWE suppressed compound 48/80-induced systemic allergic reaction and serum histamine release in mice and IgE-mediated local allergic reactions .
	manualset3
222937	4	420818	7	NULL	NULL	NULL	NULL	serum histamine release	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , LOWE suppressed compound 48/80-induced systemic allergic reaction and serum histamine release in mice and IgE-mediated local allergic reactions .
	manualset3
222938	5	420818	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , LOWE suppressed compound 48/80-induced systemic allergic reaction and serum histamine release in mice and IgE-mediated local allergic reactions .
	manualset3
222939	6	420818	7	NULL	NULL	0	NULL	IgE-mediated local allergic reactions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , LOWE suppressed compound 48/80-induced systemic allergic reaction and serum histamine release in mice and IgE-mediated local allergic reactions .
	manualset3
222940	1	420819	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of solid phase extraction ( SPE ) enhanced the detection limit to 2 ppb mass fraction relative to lamotrigine .
	manualset3
222941	2	420819	7	NULL	NULL	0	NULL	solid phase extraction ( SPE )	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of solid phase extraction ( SPE ) enhanced the detection limit to 2 ppb mass fraction relative to lamotrigine .
	manualset3
222942	3	420819	7	NULL	NULL	0	NULL	detection limit	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of solid phase extraction ( SPE ) enhanced the detection limit to 2 ppb mass fraction relative to lamotrigine .
	manualset3
222943	4	420819	7	NULL	NULL	0	NULL	 2 ppb mass fraction	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of solid phase extraction ( SPE ) enhanced the detection limit to 2 ppb mass fraction relative to lamotrigine .
	manualset3
222944	5	420819	7	NULL	NULL	0	NULL	 lamotrigine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of solid phase extraction ( SPE ) enhanced the detection limit to 2 ppb mass fraction relative to lamotrigine .
	manualset3
222945	1	420820	7	NULL	NULL	0	NULL	self-aggregating lactobacilli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among self-aggregating lactobacilli , L. acidophilus CRL 1294 and L. salivarius CRL 1328 were able to co-aggregate with Candida spp .
	manualset3
222946	2	420820	7	NULL	NULL	0	NULL	L. acidophilus CRL 1294	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among self-aggregating lactobacilli , L. acidophilus CRL 1294 and L. salivarius CRL 1328 were able to co-aggregate with Candida spp .
	manualset3
222947	3	420820	7	NULL	NULL	0	NULL	L. salivarius CRL 1328	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among self-aggregating lactobacilli , L. acidophilus CRL 1294 and L. salivarius CRL 1328 were able to co-aggregate with Candida spp .
	manualset3
222948	4	420820	7	NULL	NULL	0	NULL	Candida spp	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among self-aggregating lactobacilli , L. acidophilus CRL 1294 and L. salivarius CRL 1328 were able to co-aggregate with Candida spp .
	manualset3
222949	1	420821	7	NULL	NULL	0	NULL	 IAk 68-83 peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The IAk 68-83 peptide inhibits antigen-dependent activation of the IAk + con-albumin restricted T cell clone D10 .
	manualset3
222950	2	420821	7	NULL	NULL	0	NULL	antigen-dependent activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The IAk 68-83 peptide inhibits antigen-dependent activation of the IAk + con-albumin restricted T cell clone D10 .
	manualset3
222951	3	420821	7	NULL	NULL	0	NULL	IAk + con-albumin restricted T cell clone D10	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The IAk 68-83 peptide inhibits antigen-dependent activation of the IAk + con-albumin restricted T cell clone D10 .
	manualset3
222952	1	420822	7	NULL	NULL	0	NULL	 reference diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A reference diet ( diet A , 42 % energy from fat , ratio of polyunsaturated to saturated fatty acids ( P : S ratio ) 0.2 ) was compared with a fat reduced diet ( diet B , 35 % energy from fat , P : S ratio 0.5 ) and with a further fat modified diet supplemented with fiber ( diet C , 27 % energy from fat , P : S ratio 1.0 ) .
	manualset3
222953	2	420822	7	NULL	NULL	0	NULL	diet A 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A reference diet ( diet A , 42 % energy from fat , ratio of polyunsaturated to saturated fatty acids ( P : S ratio ) 0.2 ) was compared with a fat reduced diet ( diet B , 35 % energy from fat , P : S ratio 0.5 ) and with a further fat modified diet supplemented with fiber ( diet C , 27 % energy from fat , P : S ratio 1.0 ) .
	manualset3
222954	3	420822	7	NULL	NULL	0	NULL	42 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A reference diet ( diet A , 42 % energy from fat , ratio of polyunsaturated to saturated fatty acids ( P : S ratio ) 0.2 ) was compared with a fat reduced diet ( diet B , 35 % energy from fat , P : S ratio 0.5 ) and with a further fat modified diet supplemented with fiber ( diet C , 27 % energy from fat , P : S ratio 1.0 ) .
	manualset3
222955	4	420822	7	NULL	NULL	0	NULL	energy	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A reference diet ( diet A , 42 % energy from fat , ratio of polyunsaturated to saturated fatty acids ( P : S ratio ) 0.2 ) was compared with a fat reduced diet ( diet B , 35 % energy from fat , P : S ratio 0.5 ) and with a further fat modified diet supplemented with fiber ( diet C , 27 % energy from fat , P : S ratio 1.0 ) .
	manualset3
222956	5	420822	7	NULL	NULL	0	NULL	fat	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A reference diet ( diet A , 42 % energy from fat , ratio of polyunsaturated to saturated fatty acids ( P : S ratio ) 0.2 ) was compared with a fat reduced diet ( diet B , 35 % energy from fat , P : S ratio 0.5 ) and with a further fat modified diet supplemented with fiber ( diet C , 27 % energy from fat , P : S ratio 1.0 ) .
	manualset3
222957	6	420822	7	NULL	NULL	0	NULL	ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A reference diet ( diet A , 42 % energy from fat , ratio of polyunsaturated to saturated fatty acids ( P : S ratio ) 0.2 ) was compared with a fat reduced diet ( diet B , 35 % energy from fat , P : S ratio 0.5 ) and with a further fat modified diet supplemented with fiber ( diet C , 27 % energy from fat , P : S ratio 1.0 ) .
	manualset3
222958	7	420822	7	NULL	NULL	0	NULL	polyunsaturated fatty acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A reference diet ( diet A , 42 % energy from fat , ratio of polyunsaturated to saturated fatty acids ( P : S ratio ) 0.2 ) was compared with a fat reduced diet ( diet B , 35 % energy from fat , P : S ratio 0.5 ) and with a further fat modified diet supplemented with fiber ( diet C , 27 % energy from fat , P : S ratio 1.0 ) .
	manualset3
222959	8	420822	7	NULL	NULL	0	NULL	saturated fatty acids 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A reference diet ( diet A , 42 % energy from fat , ratio of polyunsaturated to saturated fatty acids ( P : S ratio ) 0.2 ) was compared with a fat reduced diet ( diet B , 35 % energy from fat , P : S ratio 0.5 ) and with a further fat modified diet supplemented with fiber ( diet C , 27 % energy from fat , P : S ratio 1.0 ) .
	manualset3
222960	9	420822	7	NULL	NULL	0	NULL	P : S ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A reference diet ( diet A , 42 % energy from fat , ratio of polyunsaturated to saturated fatty acids ( P : S ratio ) 0.2 ) was compared with a fat reduced diet ( diet B , 35 % energy from fat , P : S ratio 0.5 ) and with a further fat modified diet supplemented with fiber ( diet C , 27 % energy from fat , P : S ratio 1.0 ) .
	manualset3
222961	10	420822	7	NULL	NULL	0	NULL	0.2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A reference diet ( diet A , 42 % energy from fat , ratio of polyunsaturated to saturated fatty acids ( P : S ratio ) 0.2 ) was compared with a fat reduced diet ( diet B , 35 % energy from fat , P : S ratio 0.5 ) and with a further fat modified diet supplemented with fiber ( diet C , 27 % energy from fat , P : S ratio 1.0 ) .
	manualset3
222962	11	420822	7	NULL	NULL	0	NULL	fat reduced diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A reference diet ( diet A , 42 % energy from fat , ratio of polyunsaturated to saturated fatty acids ( P : S ratio ) 0.2 ) was compared with a fat reduced diet ( diet B , 35 % energy from fat , P : S ratio 0.5 ) and with a further fat modified diet supplemented with fiber ( diet C , 27 % energy from fat , P : S ratio 1.0 ) .
	manualset3
222963	12	420822	7	NULL	NULL	0	NULL	diet B 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A reference diet ( diet A , 42 % energy from fat , ratio of polyunsaturated to saturated fatty acids ( P : S ratio ) 0.2 ) was compared with a fat reduced diet ( diet B , 35 % energy from fat , P : S ratio 0.5 ) and with a further fat modified diet supplemented with fiber ( diet C , 27 % energy from fat , P : S ratio 1.0 ) .
	manualset3
222964	13	420822	7	NULL	NULL	0	NULL	35 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A reference diet ( diet A , 42 % energy from fat , ratio of polyunsaturated to saturated fatty acids ( P : S ratio ) 0.2 ) was compared with a fat reduced diet ( diet B , 35 % energy from fat , P : S ratio 0.5 ) and with a further fat modified diet supplemented with fiber ( diet C , 27 % energy from fat , P : S ratio 1.0 ) .
	manualset3
222965	14	420822	7	NULL	NULL	0	NULL	energy	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A reference diet ( diet A , 42 % energy from fat , ratio of polyunsaturated to saturated fatty acids ( P : S ratio ) 0.2 ) was compared with a fat reduced diet ( diet B , 35 % energy from fat , P : S ratio 0.5 ) and with a further fat modified diet supplemented with fiber ( diet C , 27 % energy from fat , P : S ratio 1.0 ) .
	manualset3
222966	15	420822	7	NULL	NULL	0	NULL	fat	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A reference diet ( diet A , 42 % energy from fat , ratio of polyunsaturated to saturated fatty acids ( P : S ratio ) 0.2 ) was compared with a fat reduced diet ( diet B , 35 % energy from fat , P : S ratio 0.5 ) and with a further fat modified diet supplemented with fiber ( diet C , 27 % energy from fat , P : S ratio 1.0 ) .
	manualset3
222967	16	420822	7	NULL	NULL	0	NULL	P : S ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A reference diet ( diet A , 42 % energy from fat , ratio of polyunsaturated to saturated fatty acids ( P : S ratio ) 0.2 ) was compared with a fat reduced diet ( diet B , 35 % energy from fat , P : S ratio 0.5 ) and with a further fat modified diet supplemented with fiber ( diet C , 27 % energy from fat , P : S ratio 1.0 ) .
	manualset3
222968	17	420822	7	NULL	NULL	0	NULL	0.5 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A reference diet ( diet A , 42 % energy from fat , ratio of polyunsaturated to saturated fatty acids ( P : S ratio ) 0.2 ) was compared with a fat reduced diet ( diet B , 35 % energy from fat , P : S ratio 0.5 ) and with a further fat modified diet supplemented with fiber ( diet C , 27 % energy from fat , P : S ratio 1.0 ) .
	manualset3
222969	18	420822	7	NULL	NULL	0	NULL	fat modified diet 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A reference diet ( diet A , 42 % energy from fat , ratio of polyunsaturated to saturated fatty acids ( P : S ratio ) 0.2 ) was compared with a fat reduced diet ( diet B , 35 % energy from fat , P : S ratio 0.5 ) and with a further fat modified diet supplemented with fiber ( diet C , 27 % energy from fat , P : S ratio 1.0 ) .
	manualset3
222970	19	420822	7	NULL	NULL	0	NULL	fiber	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A reference diet ( diet A , 42 % energy from fat , ratio of polyunsaturated to saturated fatty acids ( P : S ratio ) 0.2 ) was compared with a fat reduced diet ( diet B , 35 % energy from fat , P : S ratio 0.5 ) and with a further fat modified diet supplemented with fiber ( diet C , 27 % energy from fat , P : S ratio 1.0 ) .
	manualset3
222971	20	420822	7	NULL	NULL	0	NULL	 diet C	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	A reference diet ( diet A , 42 % energy from fat , ratio of polyunsaturated to saturated fatty acids ( P : S ratio ) 0.2 ) was compared with a fat reduced diet ( diet B , 35 % energy from fat , P : S ratio 0.5 ) and with a further fat modified diet supplemented with fiber ( diet C , 27 % energy from fat , P : S ratio 1.0 ) .
	manualset3
222972	21	420822	7	NULL	NULL	0	NULL	27 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A reference diet ( diet A , 42 % energy from fat , ratio of polyunsaturated to saturated fatty acids ( P : S ratio ) 0.2 ) was compared with a fat reduced diet ( diet B , 35 % energy from fat , P : S ratio 0.5 ) and with a further fat modified diet supplemented with fiber ( diet C , 27 % energy from fat , P : S ratio 1.0 ) .
	manualset3
222973	22	420822	7	NULL	NULL	0	NULL	energy	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A reference diet ( diet A , 42 % energy from fat , ratio of polyunsaturated to saturated fatty acids ( P : S ratio ) 0.2 ) was compared with a fat reduced diet ( diet B , 35 % energy from fat , P : S ratio 0.5 ) and with a further fat modified diet supplemented with fiber ( diet C , 27 % energy from fat , P : S ratio 1.0 ) .
	manualset3
222974	23	420822	7	NULL	NULL	0	NULL	fat	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A reference diet ( diet A , 42 % energy from fat , ratio of polyunsaturated to saturated fatty acids ( P : S ratio ) 0.2 ) was compared with a fat reduced diet ( diet B , 35 % energy from fat , P : S ratio 0.5 ) and with a further fat modified diet supplemented with fiber ( diet C , 27 % energy from fat , P : S ratio 1.0 ) .
	manualset3
222975	24	420822	7	NULL	NULL	0	NULL	P : S ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A reference diet ( diet A , 42 % energy from fat , ratio of polyunsaturated to saturated fatty acids ( P : S ratio ) 0.2 ) was compared with a fat reduced diet ( diet B , 35 % energy from fat , P : S ratio 0.5 ) and with a further fat modified diet supplemented with fiber ( diet C , 27 % energy from fat , P : S ratio 1.0 ) .
	manualset3
222976	25	420822	7	NULL	NULL	0	NULL	1.0 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	A reference diet ( diet A , 42 % energy from fat , ratio of polyunsaturated to saturated fatty acids ( P : S ratio ) 0.2 ) was compared with a fat reduced diet ( diet B , 35 % energy from fat , P : S ratio 0.5 ) and with a further fat modified diet supplemented with fiber ( diet C , 27 % energy from fat , P : S ratio 1.0 ) .
	manualset3
222977	1	420823	7	NULL	NULL	0	NULL	PD-1 ligands	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We found that the PD-1 ligands PD-L1 and PD-L2 were upregulated on GC B cells .
	manualset3
222978	2	420823	7	NULL	NULL	0	NULL	PD-L1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We found that the PD-1 ligands PD-L1 and PD-L2 were upregulated on GC B cells .
	manualset3
222979	3	420823	7	NULL	NULL	0	NULL	PD-L2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We found that the PD-1 ligands PD-L1 and PD-L2 were upregulated on GC B cells .
	manualset3
222980	4	420823	7	NULL	NULL	0	NULL	GC B cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We found that the PD-1 ligands PD-L1 and PD-L2 were upregulated on GC B cells .
	manualset3
222981	1	420824	7	NULL	NULL	0	NULL	Cross-reactive antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Cross-reactive antibodies were isolated by column absorption of EF-binding antibodies from LF immune sera and by column absorption of LF-binding antibodies from EF immune sera .
	manualset3
222982	2	420824	7	NULL	NULL	0	NULL	column absorption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Cross-reactive antibodies were isolated by column absorption of EF-binding antibodies from LF immune sera and by column absorption of LF-binding antibodies from EF immune sera .
	manualset3
222983	3	420824	7	NULL	NULL	0	NULL	EF-binding antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Cross-reactive antibodies were isolated by column absorption of EF-binding antibodies from LF immune sera and by column absorption of LF-binding antibodies from EF immune sera .
	manualset3
222984	4	420824	7	NULL	NULL	0	NULL	LF immune sera	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Cross-reactive antibodies were isolated by column absorption of EF-binding antibodies from LF immune sera and by column absorption of LF-binding antibodies from EF immune sera .
	manualset3
222985	5	420824	7	NULL	NULL	0	NULL	column absorption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Cross-reactive antibodies were isolated by column absorption of EF-binding antibodies from LF immune sera and by column absorption of LF-binding antibodies from EF immune sera .
	manualset3
222986	6	420824	7	NULL	NULL	0	NULL	LF-binding antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Cross-reactive antibodies were isolated by column absorption of EF-binding antibodies from LF immune sera and by column absorption of LF-binding antibodies from EF immune sera .
	manualset3
222987	7	420824	7	NULL	NULL	0	NULL	EF immune sera	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Cross-reactive antibodies were isolated by column absorption of EF-binding antibodies from LF immune sera and by column absorption of LF-binding antibodies from EF immune sera .
	manualset3
222988	1	420825	7	NULL	NULL	0	NULL	clinical history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical history of the patient , treated for bipolar affective disorder , was remarkable for transient hypothyroidism followed several months later by tremor , increased free thyroxine and triiodothyronine , and decreased TSH levels which led to lithium withdrawal .
	manualset3
222989	2	420825	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical history of the patient , treated for bipolar affective disorder , was remarkable for transient hypothyroidism followed several months later by tremor , increased free thyroxine and triiodothyronine , and decreased TSH levels which led to lithium withdrawal .
	manualset3
222990	3	420825	7	NULL	NULL	0	NULL	bipolar affective disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical history of the patient , treated for bipolar affective disorder , was remarkable for transient hypothyroidism followed several months later by tremor , increased free thyroxine and triiodothyronine , and decreased TSH levels which led to lithium withdrawal .
	manualset3
222991	4	420825	7	NULL	NULL	0	NULL	transient hypothyroidism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical history of the patient , treated for bipolar affective disorder , was remarkable for transient hypothyroidism followed several months later by tremor , increased free thyroxine and triiodothyronine , and decreased TSH levels which led to lithium withdrawal .
	manualset3
222992	5	420825	7	NULL	NULL	0	NULL	several months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical history of the patient , treated for bipolar affective disorder , was remarkable for transient hypothyroidism followed several months later by tremor , increased free thyroxine and triiodothyronine , and decreased TSH levels which led to lithium withdrawal .
	manualset3
222993	6	420825	7	NULL	NULL	0	NULL	tremor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical history of the patient , treated for bipolar affective disorder , was remarkable for transient hypothyroidism followed several months later by tremor , increased free thyroxine and triiodothyronine , and decreased TSH levels which led to lithium withdrawal .
	manualset3
222994	7	420825	7	NULL	NULL	0	NULL	free thyroxine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical history of the patient , treated for bipolar affective disorder , was remarkable for transient hypothyroidism followed several months later by tremor , increased free thyroxine and triiodothyronine , and decreased TSH levels which led to lithium withdrawal .
	manualset3
222995	8	420825	7	NULL	NULL	0	NULL	triiodothyronine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical history of the patient , treated for bipolar affective disorder , was remarkable for transient hypothyroidism followed several months later by tremor , increased free thyroxine and triiodothyronine , and decreased TSH levels which led to lithium withdrawal .
	manualset3
222996	9	420825	7	NULL	NULL	0	NULL	decreased TSH levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical history of the patient , treated for bipolar affective disorder , was remarkable for transient hypothyroidism followed several months later by tremor , increased free thyroxine and triiodothyronine , and decreased TSH levels which led to lithium withdrawal .
	manualset3
222997	10	420825	7	NULL	NULL	0	NULL	lithium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical history of the patient , treated for bipolar affective disorder , was remarkable for transient hypothyroidism followed several months later by tremor , increased free thyroxine and triiodothyronine , and decreased TSH levels which led to lithium withdrawal .
	manualset3
222998	1	420826	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , these cell lines derived from M059J cells provide us with a closer genetic match to M059J than M059K cells in studies to elucidate the function of DNA-PK .
	manualset3
222999	2	420826	7	NULL	NULL	0	NULL	cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , these cell lines derived from M059J cells provide us with a closer genetic match to M059J than M059K cells in studies to elucidate the function of DNA-PK .
	manualset3
223000	3	420826	7	NULL	NULL	0	NULL	M059J cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , these cell lines derived from M059J cells provide us with a closer genetic match to M059J than M059K cells in studies to elucidate the function of DNA-PK .
	manualset3
223001	4	420826	7	NULL	NULL	0	NULL	closer genetic match 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , these cell lines derived from M059J cells provide us with a closer genetic match to M059J than M059K cells in studies to elucidate the function of DNA-PK .
	manualset3
223002	5	420826	7	NULL	NULL	0	NULL	M059J cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , these cell lines derived from M059J cells provide us with a closer genetic match to M059J than M059K cells in studies to elucidate the function of DNA-PK .
	manualset3
223003	6	420826	7	NULL	NULL	0	NULL	M059K cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , these cell lines derived from M059J cells provide us with a closer genetic match to M059J than M059K cells in studies to elucidate the function of DNA-PK .
	manualset3
223004	7	420826	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , these cell lines derived from M059J cells provide us with a closer genetic match to M059J than M059K cells in studies to elucidate the function of DNA-PK .
	manualset3
223005	8	420826	7	NULL	NULL	0	NULL	 function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , these cell lines derived from M059J cells provide us with a closer genetic match to M059J than M059K cells in studies to elucidate the function of DNA-PK .
	manualset3
223006	9	420826	7	NULL	NULL	0	NULL	DNA-PK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , these cell lines derived from M059J cells provide us with a closer genetic match to M059J than M059K cells in studies to elucidate the function of DNA-PK .
	manualset3
223007	1	420827	7	NULL	NULL	0	NULL	chiral selector	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	As chiral selector l-4-hydroxyproline chemically bonded to 3 microm silica particles was used following the separation principle of ligand-exchange .
	manualset3
223008	2	420827	7	NULL	NULL	0	NULL	l-4-hydroxyproline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	As chiral selector l-4-hydroxyproline chemically bonded to 3 microm silica particles was used following the separation principle of ligand-exchange .
	manualset3
223009	3	420827	7	NULL	NULL	0	NULL	3 microm silica particles	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	As chiral selector l-4-hydroxyproline chemically bonded to 3 microm silica particles was used following the separation principle of ligand-exchange .
	manualset3
223010	4	420827	7	NULL	NULL	NULL	NULL	separation principle	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As chiral selector l-4-hydroxyproline chemically bonded to 3 microm silica particles was used following the separation principle of ligand-exchange .
	manualset3
223011	5	420827	7	NULL	NULL	0	NULL	ligand-exchange	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As chiral selector l-4-hydroxyproline chemically bonded to 3 microm silica particles was used following the separation principle of ligand-exchange .
	manualset3
223012	1	420828	7	NULL	NULL	0	NULL	Thirty minutes	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty minutes and 1 hour after the intravenous injection of the radiolabeled precursor , grain density in secretory odontoblasts and ameloblasts was not significantly above background labeling whereas dentin was actually labeled .
	manualset3
223013	2	420828	7	NULL	NULL	0	NULL	1 hour	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty minutes and 1 hour after the intravenous injection of the radiolabeled precursor , grain density in secretory odontoblasts and ameloblasts was not significantly above background labeling whereas dentin was actually labeled .
	manualset3
223014	3	420828	7	NULL	NULL	0	NULL	 intravenous injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty minutes and 1 hour after the intravenous injection of the radiolabeled precursor , grain density in secretory odontoblasts and ameloblasts was not significantly above background labeling whereas dentin was actually labeled .
	manualset3
223015	4	420828	7	NULL	NULL	0	NULL	radiolabeled precursor	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty minutes and 1 hour after the intravenous injection of the radiolabeled precursor , grain density in secretory odontoblasts and ameloblasts was not significantly above background labeling whereas dentin was actually labeled .
	manualset3
223016	5	420828	7	NULL	NULL	0	NULL	grain density 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty minutes and 1 hour after the intravenous injection of the radiolabeled precursor , grain density in secretory odontoblasts and ameloblasts was not significantly above background labeling whereas dentin was actually labeled .
	manualset3
223017	6	420828	7	NULL	NULL	0	NULL	secretory odontoblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty minutes and 1 hour after the intravenous injection of the radiolabeled precursor , grain density in secretory odontoblasts and ameloblasts was not significantly above background labeling whereas dentin was actually labeled .
	manualset3
223018	7	420828	7	NULL	NULL	0	NULL	ameloblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty minutes and 1 hour after the intravenous injection of the radiolabeled precursor , grain density in secretory odontoblasts and ameloblasts was not significantly above background labeling whereas dentin was actually labeled .
	manualset3
223019	8	420828	7	NULL	NULL	0	NULL	 background labeling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty minutes and 1 hour after the intravenous injection of the radiolabeled precursor , grain density in secretory odontoblasts and ameloblasts was not significantly above background labeling whereas dentin was actually labeled .
	manualset3
223020	9	420828	7	NULL	NULL	0	NULL	dentin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thirty minutes and 1 hour after the intravenous injection of the radiolabeled precursor , grain density in secretory odontoblasts and ameloblasts was not significantly above background labeling whereas dentin was actually labeled .
	manualset3
223021	1	420829	7	NULL	NULL	0	NULL	amidine derivatives	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Among several amidine derivatives tested by the authors against trypanosomatids ( T. cruzi , T. evansi and L. amazonensis ) the most effective compounds was defined as that with a methoxy group as substituent .
	manualset3
223022	2	420829	7	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among several amidine derivatives tested by the authors against trypanosomatids ( T. cruzi , T. evansi and L. amazonensis ) the most effective compounds was defined as that with a methoxy group as substituent .
	manualset3
223023	3	420829	7	NULL	NULL	0	NULL	trypanosomatids	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among several amidine derivatives tested by the authors against trypanosomatids ( T. cruzi , T. evansi and L. amazonensis ) the most effective compounds was defined as that with a methoxy group as substituent .
	manualset3
223024	4	420829	7	NULL	NULL	0	NULL	T. cruzi 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among several amidine derivatives tested by the authors against trypanosomatids ( T. cruzi , T. evansi and L. amazonensis ) the most effective compounds was defined as that with a methoxy group as substituent .
	manualset3
223025	5	420829	7	NULL	NULL	0	NULL	T. evansi	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among several amidine derivatives tested by the authors against trypanosomatids ( T. cruzi , T. evansi and L. amazonensis ) the most effective compounds was defined as that with a methoxy group as substituent .
	manualset3
223026	6	420829	7	NULL	NULL	0	NULL	L. amazonensis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among several amidine derivatives tested by the authors against trypanosomatids ( T. cruzi , T. evansi and L. amazonensis ) the most effective compounds was defined as that with a methoxy group as substituent .
	manualset3
223027	7	420829	7	NULL	NULL	0	NULL	most effective compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Among several amidine derivatives tested by the authors against trypanosomatids ( T. cruzi , T. evansi and L. amazonensis ) the most effective compounds was defined as that with a methoxy group as substituent .
	manualset3
223028	8	420829	7	NULL	NULL	0	NULL	methoxy group	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Among several amidine derivatives tested by the authors against trypanosomatids ( T. cruzi , T. evansi and L. amazonensis ) the most effective compounds was defined as that with a methoxy group as substituent .
	manualset3
223029	9	420829	7	NULL	NULL	0	NULL	substituent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Among several amidine derivatives tested by the authors against trypanosomatids ( T. cruzi , T. evansi and L. amazonensis ) the most effective compounds was defined as that with a methoxy group as substituent .
	manualset3
223030	1	420830	7	NULL	NULL	0	NULL	protein retention	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It may be concluded that protein retention was better while fat retention was nearly unaffected .
	manualset3
223031	2	420830	7	NULL	NULL	0	NULL	fat retention	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It may be concluded that protein retention was better while fat retention was nearly unaffected .
	manualset3
223032	1	420831	7	NULL	NULL	0	NULL	Direct plant tissue analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct plant tissue analysis and imprint imaging by desorption electrospray ionization mass spectrometry .
	manualset3
223033	2	420831	7	NULL	NULL	0	NULL	imprint imaging	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct plant tissue analysis and imprint imaging by desorption electrospray ionization mass spectrometry .
	manualset3
223034	3	420831	7	NULL	NULL	0	NULL	desorption electrospray ionization mass spectrometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct plant tissue analysis and imprint imaging by desorption electrospray ionization mass spectrometry .
	manualset3
223246	1	420832	7	NULL	NULL	0	NULL	depletion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Depletion of intracellular Zn ( 2 + ) with the membrane-permeant chelator N , N , N ' , N ' - tetrakis ( 2-pyridylmethyl ) - ethylenediamine ( TPEN ) resulted in the complete loss of punctate zinquin labeling .
	manualset3
223247	2	420832	7	NULL	NULL	0	NULL	intracellular Zn ( 2 + )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Depletion of intracellular Zn ( 2 + ) with the membrane-permeant chelator N , N , N ' , N ' - tetrakis ( 2-pyridylmethyl ) - ethylenediamine ( TPEN ) resulted in the complete loss of punctate zinquin labeling .
	manualset3
223248	3	420832	7	NULL	NULL	0	NULL	membrane-permeant chelator	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Depletion of intracellular Zn ( 2 + ) with the membrane-permeant chelator N , N , N ' , N ' - tetrakis ( 2-pyridylmethyl ) - ethylenediamine ( TPEN ) resulted in the complete loss of punctate zinquin labeling .
	manualset3
223249	4	420832	7	NULL	NULL	0	NULL	N , N , N ' , N ' - tetrakis ( 2-pyridylmethyl ) - ethylenediamine ( TPEN )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Depletion of intracellular Zn ( 2 + ) with the membrane-permeant chelator N , N , N ' , N ' - tetrakis ( 2-pyridylmethyl ) - ethylenediamine ( TPEN ) resulted in the complete loss of punctate zinquin labeling .
	manualset3
223250	5	420832	7	NULL	NULL	0	NULL	complete loss	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Depletion of intracellular Zn ( 2 + ) with the membrane-permeant chelator N , N , N ' , N ' - tetrakis ( 2-pyridylmethyl ) - ethylenediamine ( TPEN ) resulted in the complete loss of punctate zinquin labeling .
	manualset3
223251	6	420832	7	NULL	NULL	0	NULL	punctate zinquin labeling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Depletion of intracellular Zn ( 2 + ) with the membrane-permeant chelator N , N , N ' , N ' - tetrakis ( 2-pyridylmethyl ) - ethylenediamine ( TPEN ) resulted in the complete loss of punctate zinquin labeling .
	manualset3
223252	1	420833	7	NULL	NULL	0	NULL	Femurs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Femurs were collected on PND 35 , 77 and 350 , and diaphysis was analyzed by peripheral quantitative computed tomography and three-point bending test , while femoral neck was assessed in an axial loading experiment .
	manualset3
223253	2	420833	7	NULL	NULL	0	NULL	PND 35	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Femurs were collected on PND 35 , 77 and 350 , and diaphysis was analyzed by peripheral quantitative computed tomography and three-point bending test , while femoral neck was assessed in an axial loading experiment .
	manualset3
223254	3	420833	7	NULL	NULL	0	NULL	PND 77	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Femurs were collected on PND 35 , 77 and 350 , and diaphysis was analyzed by peripheral quantitative computed tomography and three-point bending test , while femoral neck was assessed in an axial loading experiment .
	manualset3
223255	4	420833	7	NULL	NULL	0	NULL	PND 350	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Femurs were collected on PND 35 , 77 and 350 , and diaphysis was analyzed by peripheral quantitative computed tomography and three-point bending test , while femoral neck was assessed in an axial loading experiment .
	manualset3
223256	5	420833	7	NULL	NULL	0	NULL	 diaphysis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Femurs were collected on PND 35 , 77 and 350 , and diaphysis was analyzed by peripheral quantitative computed tomography and three-point bending test , while femoral neck was assessed in an axial loading experiment .
	manualset3
223257	6	420833	7	NULL	NULL	NULL	NULL	peripheral quantitative computed tomography	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Femurs were collected on PND 35 , 77 and 350 , and diaphysis was analyzed by peripheral quantitative computed tomography and three-point bending test , while femoral neck was assessed in an axial loading experiment .
	manualset3
223258	7	420833	7	NULL	NULL	NULL	NULL	three-point bending test 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Femurs were collected on PND 35 , 77 and 350 , and diaphysis was analyzed by peripheral quantitative computed tomography and three-point bending test , while femoral neck was assessed in an axial loading experiment .
	manualset3
223259	8	420833	7	NULL	NULL	0	NULL	femoral neck	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Femurs were collected on PND 35 , 77 and 350 , and diaphysis was analyzed by peripheral quantitative computed tomography and three-point bending test , while femoral neck was assessed in an axial loading experiment .
	manualset3
223260	9	420833	7	NULL	NULL	0	NULL	axial loading experiment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Femurs were collected on PND 35 , 77 and 350 , and diaphysis was analyzed by peripheral quantitative computed tomography and three-point bending test , while femoral neck was assessed in an axial loading experiment .
	manualset3
223261	1	420834	7	NULL	NULL	0	NULL	 tumor suppressor PTEN	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The tumor suppressor PTEN is a dual protein and phosphoinositide phosphatase that negatively controls the phosphatidylinositol ( PI ) 3-kinase/protein kinase B ( Akt/PKB ) signaling pathway .
	manualset3
223262	2	420834	7	NULL	NULL	0	NULL	dual protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The tumor suppressor PTEN is a dual protein and phosphoinositide phosphatase that negatively controls the phosphatidylinositol ( PI ) 3-kinase/protein kinase B ( Akt/PKB ) signaling pathway .
	manualset3
223263	3	420834	7	NULL	NULL	0	NULL	phosphoinositide phosphatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The tumor suppressor PTEN is a dual protein and phosphoinositide phosphatase that negatively controls the phosphatidylinositol ( PI ) 3-kinase/protein kinase B ( Akt/PKB ) signaling pathway .
	manualset3
223264	4	420834	7	NULL	NULL	0	NULL	phosphatidylinositol ( PI ) 3-kinase/protein kinase B ( Akt/PKB ) signaling pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The tumor suppressor PTEN is a dual protein and phosphoinositide phosphatase that negatively controls the phosphatidylinositol ( PI ) 3-kinase/protein kinase B ( Akt/PKB ) signaling pathway .
	manualset3
223265	1	420835	7	NULL	NULL	0	NULL	ABR	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We conclude , however , that the ABR can be applied in early detection of auditory deficit .
	manualset3
223266	2	420835	7	NULL	NULL	0	NULL	early detection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We conclude , however , that the ABR can be applied in early detection of auditory deficit .
	manualset3
223267	3	420835	7	NULL	NULL	0	NULL	auditory deficit	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We conclude , however , that the ABR can be applied in early detection of auditory deficit .
	manualset3
223268	1	420836	7	NULL	NULL	0	NULL	No abnormal deposits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No abnormal deposits of immune globulins or complement were found in this specimen .
	manualset3
223269	2	420836	7	NULL	NULL	0	NULL	immune globulins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No abnormal deposits of immune globulins or complement were found in this specimen .
	manualset3
223270	3	420836	7	NULL	NULL	0	NULL	complement	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No abnormal deposits of immune globulins or complement were found in this specimen .
	manualset3
223271	4	420836	7	NULL	NULL	0	NULL	specimen	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	No abnormal deposits of immune globulins or complement were found in this specimen .
	manualset3
223272	1	420837	7	NULL	NULL	0	NULL	PRINCIPLES	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	PRINCIPLES OF TOPICAL TREATMENT OF OTITIS EXTERNA AND OTITIS MEDIA , AND A REPORT OF A CLINICAL STUDY .
	manualset3
223273	2	420837	7	NULL	NULL	0	NULL	TOPICAL TREATMENT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	PRINCIPLES OF TOPICAL TREATMENT OF OTITIS EXTERNA AND OTITIS MEDIA , AND A REPORT OF A CLINICAL STUDY .
	manualset3
223274	3	420837	7	NULL	NULL	0	NULL	OTITIS EXTERNA	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	PRINCIPLES OF TOPICAL TREATMENT OF OTITIS EXTERNA AND OTITIS MEDIA , AND A REPORT OF A CLINICAL STUDY .
	manualset3
223275	4	420837	7	NULL	NULL	0	NULL	OTITIS MEDIA	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	PRINCIPLES OF TOPICAL TREATMENT OF OTITIS EXTERNA AND OTITIS MEDIA , AND A REPORT OF A CLINICAL STUDY .
	manualset3
223276	5	420837	7	NULL	NULL	0	NULL	REPORT	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	PRINCIPLES OF TOPICAL TREATMENT OF OTITIS EXTERNA AND OTITIS MEDIA , AND A REPORT OF A CLINICAL STUDY .
	manualset3
223277	6	420837	7	NULL	NULL	0	NULL	CLINICAL STUDY	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	PRINCIPLES OF TOPICAL TREATMENT OF OTITIS EXTERNA AND OTITIS MEDIA , AND A REPORT OF A CLINICAL STUDY .
	manualset3
223278	1	420838	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , they showed an inverse correlation with nonprotein sulfhydryl ( NPSH ) levels in whole blood .
	manualset3
223279	2	420838	7	NULL	NULL	0	NULL	 inverse correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , they showed an inverse correlation with nonprotein sulfhydryl ( NPSH ) levels in whole blood .
	manualset3
223280	3	420838	7	NULL	NULL	0	NULL	nonprotein sulfhydryl ( NPSH ) levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , they showed an inverse correlation with nonprotein sulfhydryl ( NPSH ) levels in whole blood .
	manualset3
223281	4	420838	7	NULL	NULL	0	NULL	whole blood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , they showed an inverse correlation with nonprotein sulfhydryl ( NPSH ) levels in whole blood .
	manualset3
223282	1	420839	7	NULL	NULL	0	NULL	CC chemokine expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We examined CC chemokine expression in the CNS throughout the entire course of the disease and found that the production of macrophage inflammatory protein ( MIP ) -1 alpha correlated with increasing acute disease severity and remained elevated throughout chronic , relapsing disease .
	manualset3
223283	2	420839	7	NULL	NULL	0	NULL	CNS	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We examined CC chemokine expression in the CNS throughout the entire course of the disease and found that the production of macrophage inflammatory protein ( MIP ) -1 alpha correlated with increasing acute disease severity and remained elevated throughout chronic , relapsing disease .
	manualset3
223284	3	420839	7	NULL	NULL	0	NULL	entire course	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We examined CC chemokine expression in the CNS throughout the entire course of the disease and found that the production of macrophage inflammatory protein ( MIP ) -1 alpha correlated with increasing acute disease severity and remained elevated throughout chronic , relapsing disease .
	manualset3
223285	4	420839	7	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We examined CC chemokine expression in the CNS throughout the entire course of the disease and found that the production of macrophage inflammatory protein ( MIP ) -1 alpha correlated with increasing acute disease severity and remained elevated throughout chronic , relapsing disease .
	manualset3
223286	5	420839	7	NULL	NULL	0	NULL	production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We examined CC chemokine expression in the CNS throughout the entire course of the disease and found that the production of macrophage inflammatory protein ( MIP ) -1 alpha correlated with increasing acute disease severity and remained elevated throughout chronic , relapsing disease .
	manualset3
223287	6	420839	7	NULL	NULL	0	NULL	macrophage inflammatory protein ( MIP ) -1 alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We examined CC chemokine expression in the CNS throughout the entire course of the disease and found that the production of macrophage inflammatory protein ( MIP ) -1 alpha correlated with increasing acute disease severity and remained elevated throughout chronic , relapsing disease .
	manualset3
223288	7	420839	7	NULL	NULL	0	NULL	acute disease severity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We examined CC chemokine expression in the CNS throughout the entire course of the disease and found that the production of macrophage inflammatory protein ( MIP ) -1 alpha correlated with increasing acute disease severity and remained elevated throughout chronic , relapsing disease .
	manualset3
223289	8	420839	7	NULL	NULL	0	NULL	chronic , relapsing disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We examined CC chemokine expression in the CNS throughout the entire course of the disease and found that the production of macrophage inflammatory protein ( MIP ) -1 alpha correlated with increasing acute disease severity and remained elevated throughout chronic , relapsing disease .
	manualset3
223290	1	420840	7	NULL	NULL	0	NULL	stunted adults 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among stunted adults eating no more than 66 % of the requirements ( adjusted for stature ) , overweight/obesity was 35 % in women and 25 % in men .
	manualset3
223291	2	420840	7	NULL	NULL	0	NULL	66 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among stunted adults eating no more than 66 % of the requirements ( adjusted for stature ) , overweight/obesity was 35 % in women and 25 % in men .
	manualset3
223292	3	420840	7	NULL	NULL	0	NULL	 requirements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among stunted adults eating no more than 66 % of the requirements ( adjusted for stature ) , overweight/obesity was 35 % in women and 25 % in men .
	manualset3
223293	4	420840	7	NULL	NULL	0	NULL	stature	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among stunted adults eating no more than 66 % of the requirements ( adjusted for stature ) , overweight/obesity was 35 % in women and 25 % in men .
	manualset3
223294	5	420840	7	NULL	NULL	0	NULL	overweight/obesity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among stunted adults eating no more than 66 % of the requirements ( adjusted for stature ) , overweight/obesity was 35 % in women and 25 % in men .
	manualset3
223295	6	420840	7	NULL	NULL	0	NULL	35 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among stunted adults eating no more than 66 % of the requirements ( adjusted for stature ) , overweight/obesity was 35 % in women and 25 % in men .
	manualset3
223296	7	420840	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among stunted adults eating no more than 66 % of the requirements ( adjusted for stature ) , overweight/obesity was 35 % in women and 25 % in men .
	manualset3
223297	8	420840	7	NULL	NULL	0	NULL	25 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among stunted adults eating no more than 66 % of the requirements ( adjusted for stature ) , overweight/obesity was 35 % in women and 25 % in men .
	manualset3
223298	9	420840	7	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among stunted adults eating no more than 66 % of the requirements ( adjusted for stature ) , overweight/obesity was 35 % in women and 25 % in men .
	manualset3
223299	1	420841	7	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on ( Na + plus K + ) - activated ATPase .
	manualset3
223300	2	420841	7	NULL	NULL	0	NULL	( Na + plus K + ) - activated ATPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on ( Na + plus K + ) - activated ATPase .
	manualset3
223301	1	420842	7	NULL	NULL	0	NULL	Double-helix formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Double-helix formation of self-complementary chimeric oligonucleotides r ( CG ) nd ( CG ) 3-n ( n = 0 , 1 , 2 , 3 ) .
	manualset3
223302	2	420842	7	NULL	NULL	0	NULL	 self-complementary chimeric oligonucleotides	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Double-helix formation of self-complementary chimeric oligonucleotides r ( CG ) nd ( CG ) 3-n ( n = 0 , 1 , 2 , 3 ) .
	manualset3
223303	3	420842	7	NULL	NULL	0	NULL	 r ( CG ) nd ( CG ) 3-n ( n = 0 , 1 , 2 , 3 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Double-helix formation of self-complementary chimeric oligonucleotides r ( CG ) nd ( CG ) 3-n ( n = 0 , 1 , 2 , 3 ) .
	manualset3
223563	1	420843	7	NULL	NULL	0	NULL	ORF2280 proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarity with the ORF2280 proteins is restricted to a single region of about 130 amino acids that contains : ( 1 ) sequences resembling a nucleotide binding site but lacking two normally conserved residues , and ( 2 ) a downstream conserved motif with the consensus sequence VIX2TX2PX3DPALX2P .
	manualset3
223564	2	420843	7	NULL	NULL	NULL	NULL	single region	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Similarity with the ORF2280 proteins is restricted to a single region of about 130 amino acids that contains : ( 1 ) sequences resembling a nucleotide binding site but lacking two normally conserved residues , and ( 2 ) a downstream conserved motif with the consensus sequence VIX2TX2PX3DPALX2P .
	manualset3
223566	3	420843	7	NULL	NULL	NULL	NULL	130 amino acids	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Similarity with the ORF2280 proteins is restricted to a single region of about 130 amino acids that contains : ( 1 ) sequences resembling a nucleotide binding site but lacking two normally conserved residues , and ( 2 ) a downstream conserved motif with the consensus sequence VIX2TX2PX3DPALX2P .
	manualset3
223570	4	420843	7	NULL	NULL	0	NULL	 sequences	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarity with the ORF2280 proteins is restricted to a single region of about 130 amino acids that contains : ( 1 ) sequences resembling a nucleotide binding site but lacking two normally conserved residues , and ( 2 ) a downstream conserved motif with the consensus sequence VIX2TX2PX3DPALX2P .
	manualset3
223573	5	420843	7	NULL	NULL	0	NULL	nucleotide binding site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarity with the ORF2280 proteins is restricted to a single region of about 130 amino acids that contains : ( 1 ) sequences resembling a nucleotide binding site but lacking two normally conserved residues , and ( 2 ) a downstream conserved motif with the consensus sequence VIX2TX2PX3DPALX2P .
	manualset3
223574	6	420843	7	NULL	NULL	0	NULL	conserved residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarity with the ORF2280 proteins is restricted to a single region of about 130 amino acids that contains : ( 1 ) sequences resembling a nucleotide binding site but lacking two normally conserved residues , and ( 2 ) a downstream conserved motif with the consensus sequence VIX2TX2PX3DPALX2P .
	manualset3
223575	7	420843	7	NULL	NULL	0	NULL	downstream conserved motif	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarity with the ORF2280 proteins is restricted to a single region of about 130 amino acids that contains : ( 1 ) sequences resembling a nucleotide binding site but lacking two normally conserved residues , and ( 2 ) a downstream conserved motif with the consensus sequence VIX2TX2PX3DPALX2P .
	manualset3
223579	8	420843	7	NULL	NULL	0	NULL	consensus sequence VIX2TX2PX3DPALX2P	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarity with the ORF2280 proteins is restricted to a single region of about 130 amino acids that contains : ( 1 ) sequences resembling a nucleotide binding site but lacking two normally conserved residues , and ( 2 ) a downstream conserved motif with the consensus sequence VIX2TX2PX3DPALX2P .
	manualset3
223585	1	420844	7	NULL	NULL	0	NULL	Correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between the higher structure and biological functions of lentinan , a beta-1 , 6 ; 1 , 3-glucan capable of potentiating T - and non-T-cell-mediated responses , were investigated by measurements of optical rotation and some biological responses .
	manualset3
223588	2	420844	7	NULL	NULL	0	NULL	 higher structure 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between the higher structure and biological functions of lentinan , a beta-1 , 6 ; 1 , 3-glucan capable of potentiating T - and non-T-cell-mediated responses , were investigated by measurements of optical rotation and some biological responses .
	manualset3
223592	3	420844	7	NULL	NULL	0	NULL	biological functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between the higher structure and biological functions of lentinan , a beta-1 , 6 ; 1 , 3-glucan capable of potentiating T - and non-T-cell-mediated responses , were investigated by measurements of optical rotation and some biological responses .
	manualset3
223593	4	420844	7	NULL	NULL	0	NULL	lentinan	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between the higher structure and biological functions of lentinan , a beta-1 , 6 ; 1 , 3-glucan capable of potentiating T - and non-T-cell-mediated responses , were investigated by measurements of optical rotation and some biological responses .
	manualset3
223594	5	420844	7	NULL	NULL	0	NULL	beta-1 , 6 ; 1 , 3-glucan	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between the higher structure and biological functions of lentinan , a beta-1 , 6 ; 1 , 3-glucan capable of potentiating T - and non-T-cell-mediated responses , were investigated by measurements of optical rotation and some biological responses .
	manualset3
223596	6	420844	7	NULL	NULL	0	NULL	T - cell-mediated responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between the higher structure and biological functions of lentinan , a beta-1 , 6 ; 1 , 3-glucan capable of potentiating T - and non-T-cell-mediated responses , were investigated by measurements of optical rotation and some biological responses .
	manualset3
223597	7	420844	7	NULL	NULL	0	NULL	 non-T-cell-mediated responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between the higher structure and biological functions of lentinan , a beta-1 , 6 ; 1 , 3-glucan capable of potentiating T - and non-T-cell-mediated responses , were investigated by measurements of optical rotation and some biological responses .
	manualset3
223598	8	420844	7	NULL	NULL	0	NULL	measurements 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between the higher structure and biological functions of lentinan , a beta-1 , 6 ; 1 , 3-glucan capable of potentiating T - and non-T-cell-mediated responses , were investigated by measurements of optical rotation and some biological responses .
	manualset3
223599	9	420844	7	NULL	NULL	0	NULL	optical rotation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between the higher structure and biological functions of lentinan , a beta-1 , 6 ; 1 , 3-glucan capable of potentiating T - and non-T-cell-mediated responses , were investigated by measurements of optical rotation and some biological responses .
	manualset3
223600	10	420844	7	NULL	NULL	0	NULL	biological responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between the higher structure and biological functions of lentinan , a beta-1 , 6 ; 1 , 3-glucan capable of potentiating T - and non-T-cell-mediated responses , were investigated by measurements of optical rotation and some biological responses .
	manualset3
223607	1	420845	7	NULL	NULL	0	NULL	Reduced expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced expression of Shh and Bmp2 indicates that a smaller `` incisor field '' forms in Pax9 ( + / - ) ; Msx1 ( + / - ) mutants , and dental epithelial growth is substantially reduced after the bud to cap stage transition .
	manualset3
223610	2	420845	7	NULL	NULL	0	NULL	Shh	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced expression of Shh and Bmp2 indicates that a smaller `` incisor field '' forms in Pax9 ( + / - ) ; Msx1 ( + / - ) mutants , and dental epithelial growth is substantially reduced after the bud to cap stage transition .
	manualset3
223613	3	420845	7	NULL	NULL	0	NULL	Bmp2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced expression of Shh and Bmp2 indicates that a smaller `` incisor field '' forms in Pax9 ( + / - ) ; Msx1 ( + / - ) mutants , and dental epithelial growth is substantially reduced after the bud to cap stage transition .
	manualset3
223618	4	420845	7	NULL	NULL	0	NULL	smaller `` incisor field '' forms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced expression of Shh and Bmp2 indicates that a smaller `` incisor field '' forms in Pax9 ( + / - ) ; Msx1 ( + / - ) mutants , and dental epithelial growth is substantially reduced after the bud to cap stage transition .
	manualset3
223623	5	420845	7	NULL	NULL	0	NULL	Pax9 ( + / - ) mutants	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced expression of Shh and Bmp2 indicates that a smaller `` incisor field '' forms in Pax9 ( + / - ) ; Msx1 ( + / - ) mutants , and dental epithelial growth is substantially reduced after the bud to cap stage transition .
	manualset3
223625	6	420845	7	NULL	NULL	0	NULL	Msx1 ( + / - ) mutants	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced expression of Shh and Bmp2 indicates that a smaller `` incisor field '' forms in Pax9 ( + / - ) ; Msx1 ( + / - ) mutants , and dental epithelial growth is substantially reduced after the bud to cap stage transition .
	manualset3
223627	7	420845	7	NULL	NULL	0	NULL	dental epithelial growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced expression of Shh and Bmp2 indicates that a smaller `` incisor field '' forms in Pax9 ( + / - ) ; Msx1 ( + / - ) mutants , and dental epithelial growth is substantially reduced after the bud to cap stage transition .
	manualset3
223628	8	420845	7	NULL	NULL	0	NULL	bud 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced expression of Shh and Bmp2 indicates that a smaller `` incisor field '' forms in Pax9 ( + / - ) ; Msx1 ( + / - ) mutants , and dental epithelial growth is substantially reduced after the bud to cap stage transition .
	manualset3
223631	9	420845	7	NULL	NULL	0	NULL	cap	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced expression of Shh and Bmp2 indicates that a smaller `` incisor field '' forms in Pax9 ( + / - ) ; Msx1 ( + / - ) mutants , and dental epithelial growth is substantially reduced after the bud to cap stage transition .
	manualset3
223635	10	420845	7	NULL	NULL	0	NULL	stage transition 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced expression of Shh and Bmp2 indicates that a smaller `` incisor field '' forms in Pax9 ( + / - ) ; Msx1 ( + / - ) mutants , and dental epithelial growth is substantially reduced after the bud to cap stage transition .
	manualset3
223708	1	420846	7	NULL	NULL	0	NULL	Basal triglyceride levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Basal triglyceride levels were similar in patients and controls and rose to a similar extent in both groups during TPN .
	manualset3
223709	2	420846	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Basal triglyceride levels were similar in patients and controls and rose to a similar extent in both groups during TPN .
	manualset3
223710	3	420846	7	NULL	NULL	0	NULL	 controls	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Basal triglyceride levels were similar in patients and controls and rose to a similar extent in both groups during TPN .
	manualset3
223711	4	420846	7	NULL	NULL	0	NULL	groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Basal triglyceride levels were similar in patients and controls and rose to a similar extent in both groups during TPN .
	manualset3
223712	5	420846	7	NULL	NULL	0	NULL	 TPN	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Basal triglyceride levels were similar in patients and controls and rose to a similar extent in both groups during TPN .
	manualset3
223713	1	420847	7	NULL	NULL	0	NULL	archaeal RNA polymerase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The archaeal RNA polymerase terminated with high efficiency at the first terminator at 90 degrees C when it contained five to six T residues , at 80 degrees C readthrough was significantly increased .
	manualset3
223714	2	420847	7	NULL	NULL	0	NULL	high efficiency 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The archaeal RNA polymerase terminated with high efficiency at the first terminator at 90 degrees C when it contained five to six T residues , at 80 degrees C readthrough was significantly increased .
	manualset3
223715	3	420847	7	NULL	NULL	0	NULL	 first terminator	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The archaeal RNA polymerase terminated with high efficiency at the first terminator at 90 degrees C when it contained five to six T residues , at 80 degrees C readthrough was significantly increased .
	manualset3
223716	4	420847	7	NULL	NULL	0	NULL	90 degrees C	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The archaeal RNA polymerase terminated with high efficiency at the first terminator at 90 degrees C when it contained five to six T residues , at 80 degrees C readthrough was significantly increased .
	manualset3
223717	5	420847	7	NULL	NULL	0	NULL	five to six T residues	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The archaeal RNA polymerase terminated with high efficiency at the first terminator at 90 degrees C when it contained five to six T residues , at 80 degrees C readthrough was significantly increased .
	manualset3
223718	6	420847	7	NULL	NULL	0	NULL	80 degrees C	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The archaeal RNA polymerase terminated with high efficiency at the first terminator at 90 degrees C when it contained five to six T residues , at 80 degrees C readthrough was significantly increased .
	manualset3
223719	7	420847	7	NULL	NULL	0	NULL	readthrough	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The archaeal RNA polymerase terminated with high efficiency at the first terminator at 90 degrees C when it contained five to six T residues , at 80 degrees C readthrough was significantly increased .
	manualset3
223720	1	420849	7	NULL	NULL	0	NULL	Local treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Local treatment was surgery in 53 % of patients , surgery + radiotherapy in 25 % and radiotherapy only in 22 % .
	manualset3
223721	2	420849	7	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Local treatment was surgery in 53 % of patients , surgery + radiotherapy in 25 % and radiotherapy only in 22 % .
	manualset3
223722	3	420849	7	NULL	NULL	0	NULL	53 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Local treatment was surgery in 53 % of patients , surgery + radiotherapy in 25 % and radiotherapy only in 22 % .
	manualset3
223723	4	420849	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Local treatment was surgery in 53 % of patients , surgery + radiotherapy in 25 % and radiotherapy only in 22 % .
	manualset3
223724	5	420849	7	NULL	NULL	0	NULL	surgery + radiotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Local treatment was surgery in 53 % of patients , surgery + radiotherapy in 25 % and radiotherapy only in 22 % .
	manualset3
223725	6	420849	7	NULL	NULL	0	NULL	25 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Local treatment was surgery in 53 % of patients , surgery + radiotherapy in 25 % and radiotherapy only in 22 % .
	manualset3
223726	7	420849	7	NULL	NULL	0	NULL	radiotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Local treatment was surgery in 53 % of patients , surgery + radiotherapy in 25 % and radiotherapy only in 22 % .
	manualset3
223727	8	420849	7	NULL	NULL	0	NULL	22 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Local treatment was surgery in 53 % of patients , surgery + radiotherapy in 25 % and radiotherapy only in 22 % .
	manualset3
223728	1	420850	7	NULL	NULL	0	NULL	novel peptide ( Ainp1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We utilized a novel peptide ( Ainp1 ) to address whether the HIF-1 signaling could be suppressed by an ARNT-mediated mechanism .
	manualset3
223729	2	420850	7	NULL	NULL	0	NULL	HIF-1 signaling 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We utilized a novel peptide ( Ainp1 ) to address whether the HIF-1 signaling could be suppressed by an ARNT-mediated mechanism .
	manualset3
223730	3	420850	7	NULL	NULL	0	NULL	ARNT-mediated mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We utilized a novel peptide ( Ainp1 ) to address whether the HIF-1 signaling could be suppressed by an ARNT-mediated mechanism .
	manualset3
223731	1	420851	7	NULL	NULL	0	NULL	kinetics	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of neomycin release , in vitro , at pH = 8.2 is studied .
	manualset3
223732	2	420851	7	NULL	NULL	0	NULL	neomycin release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of neomycin release , in vitro , at pH = 8.2 is studied .
	manualset3
223733	3	420851	7	NULL	NULL	0	NULL	pH = 8.2	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The kinetics of neomycin release , in vitro , at pH = 8.2 is studied .
	manualset3
223734	1	420852	7	NULL	NULL	0	NULL	BiP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , BiP may prevent the premature escape and eventual secretion of incompletely assembled Ig molecules .
	manualset3
223735	2	420852	7	NULL	NULL	0	NULL	premature escape	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , BiP may prevent the premature escape and eventual secretion of incompletely assembled Ig molecules .
	manualset3
223736	3	420852	7	NULL	NULL	0	NULL	secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , BiP may prevent the premature escape and eventual secretion of incompletely assembled Ig molecules .
	manualset3
223737	4	420852	7	NULL	NULL	0	NULL	incompletely assembled Ig molecules	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , BiP may prevent the premature escape and eventual secretion of incompletely assembled Ig molecules .
	manualset3
223738	1	420853	7	NULL	NULL	0	NULL	test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The test of Ka/Ks ratio showed that the function of LRR was conserved because of the purifying selection , although different positions of the Rpi-blb2 LRR region were under different selection pressures .
	manualset3
223739	2	420853	7	NULL	NULL	0	NULL	Ka/Ks ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The test of Ka/Ks ratio showed that the function of LRR was conserved because of the purifying selection , although different positions of the Rpi-blb2 LRR region were under different selection pressures .
	manualset3
223740	3	420853	7	NULL	NULL	0	NULL	function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The test of Ka/Ks ratio showed that the function of LRR was conserved because of the purifying selection , although different positions of the Rpi-blb2 LRR region were under different selection pressures .
	manualset3
223741	4	420853	7	NULL	NULL	0	NULL	LRR 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The test of Ka/Ks ratio showed that the function of LRR was conserved because of the purifying selection , although different positions of the Rpi-blb2 LRR region were under different selection pressures .
	manualset3
223742	5	420853	7	NULL	NULL	0	NULL	purifying selection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The test of Ka/Ks ratio showed that the function of LRR was conserved because of the purifying selection , although different positions of the Rpi-blb2 LRR region were under different selection pressures .
	manualset3
223743	6	420853	7	NULL	NULL	0	NULL	different positions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The test of Ka/Ks ratio showed that the function of LRR was conserved because of the purifying selection , although different positions of the Rpi-blb2 LRR region were under different selection pressures .
	manualset3
223744	7	420853	7	NULL	NULL	0	NULL	Rpi-blb2 LRR region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The test of Ka/Ks ratio showed that the function of LRR was conserved because of the purifying selection , although different positions of the Rpi-blb2 LRR region were under different selection pressures .
	manualset3
223745	8	420853	7	NULL	NULL	0	NULL	selection pressures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The test of Ka/Ks ratio showed that the function of LRR was conserved because of the purifying selection , although different positions of the Rpi-blb2 LRR region were under different selection pressures .
	manualset3
223746	1	420854	7	NULL	NULL	0	NULL	procurement process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The procurement process in Italy is becoming more complex and expensive .
	manualset3
223747	2	420854	7	NULL	NULL	0	NULL	Italy	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The procurement process in Italy is becoming more complex and expensive .
	manualset3
223748	1	420855	7	NULL	NULL	0	NULL	Exendin-4	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Exendin-4 , a glucagon-like peptide-1 receptor agonist , provides neuroprotection in mice transient focal cerebral ischemia .
	manualset3
223749	2	420855	7	NULL	NULL	0	NULL	glucagon-like peptide-1 receptor agonist 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Exendin-4 , a glucagon-like peptide-1 receptor agonist , provides neuroprotection in mice transient focal cerebral ischemia .
	manualset3
223750	3	420855	7	NULL	NULL	0	NULL	 neuroprotection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Exendin-4 , a glucagon-like peptide-1 receptor agonist , provides neuroprotection in mice transient focal cerebral ischemia .
	manualset3
223751	4	420855	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Exendin-4 , a glucagon-like peptide-1 receptor agonist , provides neuroprotection in mice transient focal cerebral ischemia .
	manualset3
223752	5	420855	7	NULL	NULL	0	NULL	transient focal cerebral ischemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Exendin-4 , a glucagon-like peptide-1 receptor agonist , provides neuroprotection in mice transient focal cerebral ischemia .
	manualset3
223753	1	420856	7	NULL	NULL	0	NULL	concept	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The concept of autocrine secretion , its subsequent modifications , its application for understanding pathogenesis of disease , and its potential for developing new approaches to prevention and treatment are reviewed .
	manualset3
223754	2	420856	7	NULL	NULL	0	NULL	autocrine secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The concept of autocrine secretion , its subsequent modifications , its application for understanding pathogenesis of disease , and its potential for developing new approaches to prevention and treatment are reviewed .
	manualset3
223755	3	420856	7	NULL	NULL	0	NULL	modifications	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The concept of autocrine secretion , its subsequent modifications , its application for understanding pathogenesis of disease , and its potential for developing new approaches to prevention and treatment are reviewed .
	manualset3
223756	4	420856	7	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The concept of autocrine secretion , its subsequent modifications , its application for understanding pathogenesis of disease , and its potential for developing new approaches to prevention and treatment are reviewed .
	manualset3
223757	5	420856	7	NULL	NULL	0	NULL	understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The concept of autocrine secretion , its subsequent modifications , its application for understanding pathogenesis of disease , and its potential for developing new approaches to prevention and treatment are reviewed .
	manualset3
223758	6	420856	7	NULL	NULL	0	NULL	pathogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The concept of autocrine secretion , its subsequent modifications , its application for understanding pathogenesis of disease , and its potential for developing new approaches to prevention and treatment are reviewed .
	manualset3
223759	7	420856	7	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The concept of autocrine secretion , its subsequent modifications , its application for understanding pathogenesis of disease , and its potential for developing new approaches to prevention and treatment are reviewed .
	manualset3
223760	8	420856	7	NULL	NULL	0	NULL	new approaches	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The concept of autocrine secretion , its subsequent modifications , its application for understanding pathogenesis of disease , and its potential for developing new approaches to prevention and treatment are reviewed .
	manualset3
223761	9	420856	7	NULL	NULL	0	NULL	prevention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The concept of autocrine secretion , its subsequent modifications , its application for understanding pathogenesis of disease , and its potential for developing new approaches to prevention and treatment are reviewed .
	manualset3
223762	10	420856	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The concept of autocrine secretion , its subsequent modifications , its application for understanding pathogenesis of disease , and its potential for developing new approaches to prevention and treatment are reviewed .
	manualset3
223763	11	420856	7	NULL	NULL	0	NULL	potential	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The concept of autocrine secretion , its subsequent modifications , its application for understanding pathogenesis of disease , and its potential for developing new approaches to prevention and treatment are reviewed .
	manualset3
223764	1	420857	7	NULL	NULL	0	NULL	thirty infants 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of them , thirty infants were suffering from manifestations of gastrointestinal allergy ( patients ) and the other thirty were not suffering from such manifestations ( controls ) .
	manualset3
223765	2	420857	7	NULL	NULL	0	NULL	manifestations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Of them , thirty infants were suffering from manifestations of gastrointestinal allergy ( patients ) and the other thirty were not suffering from such manifestations ( controls ) .
	manualset3
223766	3	420857	7	NULL	NULL	0	NULL	gastrointestinal allergy 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Of them , thirty infants were suffering from manifestations of gastrointestinal allergy ( patients ) and the other thirty were not suffering from such manifestations ( controls ) .
	manualset3
223767	4	420857	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of them , thirty infants were suffering from manifestations of gastrointestinal allergy ( patients ) and the other thirty were not suffering from such manifestations ( controls ) .
	manualset3
223768	5	420857	7	NULL	NULL	0	NULL	thirty	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of them , thirty infants were suffering from manifestations of gastrointestinal allergy ( patients ) and the other thirty were not suffering from such manifestations ( controls ) .
	manualset3
223769	6	420857	7	NULL	NULL	0	NULL	manifestations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Of them , thirty infants were suffering from manifestations of gastrointestinal allergy ( patients ) and the other thirty were not suffering from such manifestations ( controls ) .
	manualset3
223770	7	420857	7	NULL	NULL	0	NULL	controls	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Of them , thirty infants were suffering from manifestations of gastrointestinal allergy ( patients ) and the other thirty were not suffering from such manifestations ( controls ) .
	manualset3
223771	1	420858	7	NULL	NULL	0	NULL	Mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice treated daily for 7-14 days with s.c. injections of TGF-beta 1 exhibited up to a 95 % reduction in circulating platelets and a 50 % reduction in red cell counts , whereas a 50 % -400 % increase occurred in circulating white cells with the morphology of small lymphocytes .
	manualset3
223772	2	420858	7	NULL	NULL	0	NULL	7-14 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice treated daily for 7-14 days with s.c. injections of TGF-beta 1 exhibited up to a 95 % reduction in circulating platelets and a 50 % reduction in red cell counts , whereas a 50 % -400 % increase occurred in circulating white cells with the morphology of small lymphocytes .
	manualset3
223773	3	420858	7	NULL	NULL	0	NULL	s.c. injections 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice treated daily for 7-14 days with s.c. injections of TGF-beta 1 exhibited up to a 95 % reduction in circulating platelets and a 50 % reduction in red cell counts , whereas a 50 % -400 % increase occurred in circulating white cells with the morphology of small lymphocytes .
	manualset3
223774	4	420858	7	NULL	NULL	0	NULL	TGF-beta 1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice treated daily for 7-14 days with s.c. injections of TGF-beta 1 exhibited up to a 95 % reduction in circulating platelets and a 50 % reduction in red cell counts , whereas a 50 % -400 % increase occurred in circulating white cells with the morphology of small lymphocytes .
	manualset3
223775	5	420858	7	NULL	NULL	0	NULL	95 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice treated daily for 7-14 days with s.c. injections of TGF-beta 1 exhibited up to a 95 % reduction in circulating platelets and a 50 % reduction in red cell counts , whereas a 50 % -400 % increase occurred in circulating white cells with the morphology of small lymphocytes .
	manualset3
223776	6	420858	7	NULL	NULL	0	NULL	reduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice treated daily for 7-14 days with s.c. injections of TGF-beta 1 exhibited up to a 95 % reduction in circulating platelets and a 50 % reduction in red cell counts , whereas a 50 % -400 % increase occurred in circulating white cells with the morphology of small lymphocytes .
	manualset3
223777	7	420858	7	NULL	NULL	0	NULL	circulating platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice treated daily for 7-14 days with s.c. injections of TGF-beta 1 exhibited up to a 95 % reduction in circulating platelets and a 50 % reduction in red cell counts , whereas a 50 % -400 % increase occurred in circulating white cells with the morphology of small lymphocytes .
	manualset3
223778	8	420858	7	NULL	NULL	0	NULL	50 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice treated daily for 7-14 days with s.c. injections of TGF-beta 1 exhibited up to a 95 % reduction in circulating platelets and a 50 % reduction in red cell counts , whereas a 50 % -400 % increase occurred in circulating white cells with the morphology of small lymphocytes .
	manualset3
223779	9	420858	7	NULL	NULL	0	NULL	reduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice treated daily for 7-14 days with s.c. injections of TGF-beta 1 exhibited up to a 95 % reduction in circulating platelets and a 50 % reduction in red cell counts , whereas a 50 % -400 % increase occurred in circulating white cells with the morphology of small lymphocytes .
	manualset3
223780	10	420858	7	NULL	NULL	0	NULL	red cell counts 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice treated daily for 7-14 days with s.c. injections of TGF-beta 1 exhibited up to a 95 % reduction in circulating platelets and a 50 % reduction in red cell counts , whereas a 50 % -400 % increase occurred in circulating white cells with the morphology of small lymphocytes .
	manualset3
223781	11	420858	7	NULL	NULL	0	NULL	50 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice treated daily for 7-14 days with s.c. injections of TGF-beta 1 exhibited up to a 95 % reduction in circulating platelets and a 50 % reduction in red cell counts , whereas a 50 % -400 % increase occurred in circulating white cells with the morphology of small lymphocytes .
	manualset3
223782	12	420858	7	NULL	NULL	0	NULL	400 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice treated daily for 7-14 days with s.c. injections of TGF-beta 1 exhibited up to a 95 % reduction in circulating platelets and a 50 % reduction in red cell counts , whereas a 50 % -400 % increase occurred in circulating white cells with the morphology of small lymphocytes .
	manualset3
223783	13	420858	7	NULL	NULL	0	NULL	circulating white cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice treated daily for 7-14 days with s.c. injections of TGF-beta 1 exhibited up to a 95 % reduction in circulating platelets and a 50 % reduction in red cell counts , whereas a 50 % -400 % increase occurred in circulating white cells with the morphology of small lymphocytes .
	manualset3
223784	14	420858	7	NULL	NULL	0	NULL	morphology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice treated daily for 7-14 days with s.c. injections of TGF-beta 1 exhibited up to a 95 % reduction in circulating platelets and a 50 % reduction in red cell counts , whereas a 50 % -400 % increase occurred in circulating white cells with the morphology of small lymphocytes .
	manualset3
223785	15	420858	7	NULL	NULL	0	NULL	small lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mice treated daily for 7-14 days with s.c. injections of TGF-beta 1 exhibited up to a 95 % reduction in circulating platelets and a 50 % reduction in red cell counts , whereas a 50 % -400 % increase occurred in circulating white cells with the morphology of small lymphocytes .
	manualset3
223786	1	420859	7	NULL	NULL	0	NULL	Human-specific loss	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Human-specific loss of regulatory DNA and the evolution of human-specific traits .
	manualset3
223787	2	420859	7	NULL	NULL	0	NULL	regulatory DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Human-specific loss of regulatory DNA and the evolution of human-specific traits .
	manualset3
223788	3	420859	7	NULL	NULL	0	NULL	evolution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Human-specific loss of regulatory DNA and the evolution of human-specific traits .
	manualset3
223789	4	420859	7	NULL	NULL	0	NULL	human-specific traits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Human-specific loss of regulatory DNA and the evolution of human-specific traits .
	manualset3
223790	1	420860	7	NULL	NULL	0	NULL	Morphology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Morphology of retinomotor response of Oncorhynchus masou fry exposed in magnetic field and red light ) .
	manualset3
223791	2	420860	7	NULL	NULL	0	NULL	retinomotor response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Morphology of retinomotor response of Oncorhynchus masou fry exposed in magnetic field and red light ) .
	manualset3
223792	3	420860	7	NULL	NULL	0	NULL	Oncorhynchus masou	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Morphology of retinomotor response of Oncorhynchus masou fry exposed in magnetic field and red light ) .
	manualset3
223793	4	420860	7	NULL	NULL	0	NULL	magnetic field 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	( Morphology of retinomotor response of Oncorhynchus masou fry exposed in magnetic field and red light ) .
	manualset3
223794	5	420860	7	NULL	NULL	0	NULL	 red light	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	( Morphology of retinomotor response of Oncorhynchus masou fry exposed in magnetic field and red light ) .
	manualset3
223795	1	420861	7	NULL	NULL	0	NULL	 present study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study synthetic salmon calcitonin ( 15 ng in 0.3 microliter ) was found to produce a marked suppression of eating when infused in several hypothalamic areas .
	manualset3
223796	2	420861	7	NULL	NULL	0	NULL	synthetic salmon calcitonin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study synthetic salmon calcitonin ( 15 ng in 0.3 microliter ) was found to produce a marked suppression of eating when infused in several hypothalamic areas .
	manualset3
223797	3	420861	7	NULL	NULL	0	NULL	15 ng	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study synthetic salmon calcitonin ( 15 ng in 0.3 microliter ) was found to produce a marked suppression of eating when infused in several hypothalamic areas .
	manualset3
223798	4	420861	7	NULL	NULL	0	NULL	0.3 microliter	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study synthetic salmon calcitonin ( 15 ng in 0.3 microliter ) was found to produce a marked suppression of eating when infused in several hypothalamic areas .
	manualset3
223799	5	420861	7	NULL	NULL	0	NULL	marked suppression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study synthetic salmon calcitonin ( 15 ng in 0.3 microliter ) was found to produce a marked suppression of eating when infused in several hypothalamic areas .
	manualset3
223800	6	420861	7	NULL	NULL	0	NULL	eating	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study synthetic salmon calcitonin ( 15 ng in 0.3 microliter ) was found to produce a marked suppression of eating when infused in several hypothalamic areas .
	manualset3
223801	7	420861	7	NULL	NULL	0	NULL	several hypothalamic areas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the present study synthetic salmon calcitonin ( 15 ng in 0.3 microliter ) was found to produce a marked suppression of eating when infused in several hypothalamic areas .
	manualset3
223802	1	420862	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This study contrasts the CT scan referring patterns of general practitioners with that of a neurologist and questions the possible overuse of this facility .
	manualset3
223803	2	420862	7	NULL	NULL	0	NULL	CT scan	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This study contrasts the CT scan referring patterns of general practitioners with that of a neurologist and questions the possible overuse of this facility .
	manualset3
223804	3	420862	7	NULL	NULL	0	NULL	patterns	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This study contrasts the CT scan referring patterns of general practitioners with that of a neurologist and questions the possible overuse of this facility .
	manualset3
223805	4	420862	7	NULL	NULL	0	NULL	 general practitioners	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This study contrasts the CT scan referring patterns of general practitioners with that of a neurologist and questions the possible overuse of this facility .
	manualset3
223806	5	420862	7	NULL	NULL	0	NULL	neurologist 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	This study contrasts the CT scan referring patterns of general practitioners with that of a neurologist and questions the possible overuse of this facility .
	manualset3
223807	6	420862	7	NULL	NULL	0	NULL	possible overuse	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This study contrasts the CT scan referring patterns of general practitioners with that of a neurologist and questions the possible overuse of this facility .
	manualset3
223808	7	420862	7	NULL	NULL	0	NULL	facility	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	This study contrasts the CT scan referring patterns of general practitioners with that of a neurologist and questions the possible overuse of this facility .
	manualset3
223809	1	420863	7	NULL	NULL	0	NULL	proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As proliferation plays a major role in pulmonary hypertension , we examined the hypothesis that angiopeptin would inhibit the development of chronic hypoxic pulmonary hypertension in the rat .
	manualset3
223810	2	420863	7	NULL	NULL	0	NULL	major role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As proliferation plays a major role in pulmonary hypertension , we examined the hypothesis that angiopeptin would inhibit the development of chronic hypoxic pulmonary hypertension in the rat .
	manualset3
223811	3	420863	7	NULL	NULL	NULL	NULL	pulmonary hypertension	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As proliferation plays a major role in pulmonary hypertension , we examined the hypothesis that angiopeptin would inhibit the development of chronic hypoxic pulmonary hypertension in the rat .
	manualset3
223812	4	420863	7	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	As proliferation plays a major role in pulmonary hypertension , we examined the hypothesis that angiopeptin would inhibit the development of chronic hypoxic pulmonary hypertension in the rat .
	manualset3
223813	5	420863	7	NULL	NULL	0	NULL	angiopeptin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	As proliferation plays a major role in pulmonary hypertension , we examined the hypothesis that angiopeptin would inhibit the development of chronic hypoxic pulmonary hypertension in the rat .
	manualset3
223814	6	420863	7	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As proliferation plays a major role in pulmonary hypertension , we examined the hypothesis that angiopeptin would inhibit the development of chronic hypoxic pulmonary hypertension in the rat .
	manualset3
223815	7	420863	7	NULL	NULL	0	NULL	chronic hypoxic pulmonary hypertension	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	As proliferation plays a major role in pulmonary hypertension , we examined the hypothesis that angiopeptin would inhibit the development of chronic hypoxic pulmonary hypertension in the rat .
	manualset3
223816	8	420863	7	NULL	NULL	0	NULL	rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	As proliferation plays a major role in pulmonary hypertension , we examined the hypothesis that angiopeptin would inhibit the development of chronic hypoxic pulmonary hypertension in the rat .
	manualset3
223817	1	420864	7	NULL	NULL	0	NULL	interventions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Various interventions that modulate pain , such as the application of a competing noxious stimulus ( counterirritation ) , are thought to involve cerebrospinal regulation through diffuse noxious inhibitory controls ( DNICs ) .
	manualset3
223818	2	420864	7	NULL	NULL	0	NULL	pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Various interventions that modulate pain , such as the application of a competing noxious stimulus ( counterirritation ) , are thought to involve cerebrospinal regulation through diffuse noxious inhibitory controls ( DNICs ) .
	manualset3
223819	3	420864	7	NULL	NULL	0	NULL	application 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Various interventions that modulate pain , such as the application of a competing noxious stimulus ( counterirritation ) , are thought to involve cerebrospinal regulation through diffuse noxious inhibitory controls ( DNICs ) .
	manualset3
223820	4	420864	7	NULL	NULL	0	NULL	competing noxious stimulus	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Various interventions that modulate pain , such as the application of a competing noxious stimulus ( counterirritation ) , are thought to involve cerebrospinal regulation through diffuse noxious inhibitory controls ( DNICs ) .
	manualset3
223821	5	420864	7	NULL	NULL	0	NULL	counterirritation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Various interventions that modulate pain , such as the application of a competing noxious stimulus ( counterirritation ) , are thought to involve cerebrospinal regulation through diffuse noxious inhibitory controls ( DNICs ) .
	manualset3
223822	6	420864	7	NULL	NULL	0	NULL	cerebrospinal regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Various interventions that modulate pain , such as the application of a competing noxious stimulus ( counterirritation ) , are thought to involve cerebrospinal regulation through diffuse noxious inhibitory controls ( DNICs ) .
	manualset3
223823	7	420864	7	NULL	NULL	0	NULL	diffuse noxious inhibitory controls ( DNICs ) 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Various interventions that modulate pain , such as the application of a competing noxious stimulus ( counterirritation ) , are thought to involve cerebrospinal regulation through diffuse noxious inhibitory controls ( DNICs ) .
	manualset3
223824	1	420865	7	NULL	NULL	0	NULL	 method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The method allows for subsequent analysis of the absorped proteins by two dimensional microelectrophoresis .
	manualset3
223825	2	420865	7	NULL	NULL	0	NULL	subsequent analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method allows for subsequent analysis of the absorped proteins by two dimensional microelectrophoresis .
	manualset3
223826	3	420865	7	NULL	NULL	0	NULL	absorped proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The method allows for subsequent analysis of the absorped proteins by two dimensional microelectrophoresis .
	manualset3
223827	4	420865	7	NULL	NULL	0	NULL	two dimensional microelectrophoresis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method allows for subsequent analysis of the absorped proteins by two dimensional microelectrophoresis .
	manualset3
223828	1	420866	7	NULL	NULL	0	NULL	23 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the 23 patients assayed as to serum CA125 level before the second-look , 18 ( 78 % ) were within normal limits ( less than 65 U/ml ) , including 12 patients ( 66.6 % ) who were second-look positive and 6 who were negative .
	manualset3
223829	2	420866	7	NULL	NULL	0	NULL	serum CA125 level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the 23 patients assayed as to serum CA125 level before the second-look , 18 ( 78 % ) were within normal limits ( less than 65 U/ml ) , including 12 patients ( 66.6 % ) who were second-look positive and 6 who were negative .
	manualset3
223830	3	420866	7	NULL	NULL	0	NULL	18 ( 78 % ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the 23 patients assayed as to serum CA125 level before the second-look , 18 ( 78 % ) were within normal limits ( less than 65 U/ml ) , including 12 patients ( 66.6 % ) who were second-look positive and 6 who were negative .
	manualset3
223831	4	420866	7	NULL	NULL	0	NULL	normal limits	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the 23 patients assayed as to serum CA125 level before the second-look , 18 ( 78 % ) were within normal limits ( less than 65 U/ml ) , including 12 patients ( 66.6 % ) who were second-look positive and 6 who were negative .
	manualset3
223832	5	420866	7	NULL	NULL	0	NULL	65 U/ml	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the 23 patients assayed as to serum CA125 level before the second-look , 18 ( 78 % ) were within normal limits ( less than 65 U/ml ) , including 12 patients ( 66.6 % ) who were second-look positive and 6 who were negative .
	manualset3
223833	6	420866	7	NULL	NULL	0	NULL	12 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the 23 patients assayed as to serum CA125 level before the second-look , 18 ( 78 % ) were within normal limits ( less than 65 U/ml ) , including 12 patients ( 66.6 % ) who were second-look positive and 6 who were negative .
	manualset3
223834	7	420866	7	NULL	NULL	0	NULL	66.6 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the 23 patients assayed as to serum CA125 level before the second-look , 18 ( 78 % ) were within normal limits ( less than 65 U/ml ) , including 12 patients ( 66.6 % ) who were second-look positive and 6 who were negative .
	manualset3
223835	8	420866	7	NULL	NULL	0	NULL	 positive	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the 23 patients assayed as to serum CA125 level before the second-look , 18 ( 78 % ) were within normal limits ( less than 65 U/ml ) , including 12 patients ( 66.6 % ) who were second-look positive and 6 who were negative .
	manualset3
223836	9	420866	7	NULL	NULL	0	NULL	6 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the 23 patients assayed as to serum CA125 level before the second-look , 18 ( 78 % ) were within normal limits ( less than 65 U/ml ) , including 12 patients ( 66.6 % ) who were second-look positive and 6 who were negative .
	manualset3
223838	10	420866	7	NULL	NULL	0	NULL	negative	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the 23 patients assayed as to serum CA125 level before the second-look , 18 ( 78 % ) were within normal limits ( less than 65 U/ml ) , including 12 patients ( 66.6 % ) who were second-look positive and 6 who were negative .
	manualset3
223839	1	420867	7	NULL	NULL	0	NULL	high-intensity ELF MFs 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The high-intensity ELF MFs ( 14 mT at power frequency ) did not act as a general stress factor .
	manualset3
223840	2	420867	7	NULL	NULL	0	NULL	14 mT	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The high-intensity ELF MFs ( 14 mT at power frequency ) did not act as a general stress factor .
	manualset3
223841	3	420867	7	NULL	NULL	0	NULL	power frequency 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The high-intensity ELF MFs ( 14 mT at power frequency ) did not act as a general stress factor .
	manualset3
223842	4	420867	7	NULL	NULL	0	NULL	general stress factor	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The high-intensity ELF MFs ( 14 mT at power frequency ) did not act as a general stress factor .
	manualset3
223843	1	420868	7	NULL	NULL	0	NULL	method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is validated by measurements with an artificial model .
	manualset3
223844	2	420868	7	NULL	NULL	0	NULL	measurements	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is validated by measurements with an artificial model .
	manualset3
223845	3	420868	7	NULL	NULL	0	NULL	artificial model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is validated by measurements with an artificial model .
	manualset3
223846	1	420869	7	NULL	NULL	0	NULL	Retrospective self-reports	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Retrospective self-reports about prior sober and alcohol intoxicated states were explored to reveal moderating effects of trait anger and alcohol consumption on anger control .
	manualset3
223847	2	420869	7	NULL	NULL	0	NULL	alcohol intoxicated states	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Retrospective self-reports about prior sober and alcohol intoxicated states were explored to reveal moderating effects of trait anger and alcohol consumption on anger control .
	manualset3
223848	3	420869	7	NULL	NULL	0	NULL	moderating effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Retrospective self-reports about prior sober and alcohol intoxicated states were explored to reveal moderating effects of trait anger and alcohol consumption on anger control .
	manualset3
223849	4	420869	7	NULL	NULL	0	NULL	anger	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Retrospective self-reports about prior sober and alcohol intoxicated states were explored to reveal moderating effects of trait anger and alcohol consumption on anger control .
	manualset3
223850	5	420869	7	NULL	NULL	NULL	NULL	alcohol consumption	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Retrospective self-reports about prior sober and alcohol intoxicated states were explored to reveal moderating effects of trait anger and alcohol consumption on anger control .
	manualset3
223851	6	420869	7	NULL	NULL	0	NULL	anger control	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Retrospective self-reports about prior sober and alcohol intoxicated states were explored to reveal moderating effects of trait anger and alcohol consumption on anger control .
	manualset3
223852	1	420870	7	NULL	NULL	0	NULL	Focusing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Focusing on symptoms of attention deficit hyperactivity disorder ( ADHD ) in a sample obtained from the general population , we aimed to investigate the effects of incentives and event rate on reaction time ( RT ) performance and response inhibition .
	manualset3
223853	2	420870	7	NULL	NULL	0	NULL	symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Focusing on symptoms of attention deficit hyperactivity disorder ( ADHD ) in a sample obtained from the general population , we aimed to investigate the effects of incentives and event rate on reaction time ( RT ) performance and response inhibition .
	manualset3
223854	3	420870	7	NULL	NULL	0	NULL	attention deficit hyperactivity disorder ( ADHD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Focusing on symptoms of attention deficit hyperactivity disorder ( ADHD ) in a sample obtained from the general population , we aimed to investigate the effects of incentives and event rate on reaction time ( RT ) performance and response inhibition .
	manualset3
223855	4	420870	7	NULL	NULL	0	NULL	sample	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Focusing on symptoms of attention deficit hyperactivity disorder ( ADHD ) in a sample obtained from the general population , we aimed to investigate the effects of incentives and event rate on reaction time ( RT ) performance and response inhibition .
	manualset3
223856	5	420870	7	NULL	NULL	0	NULL	general population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Focusing on symptoms of attention deficit hyperactivity disorder ( ADHD ) in a sample obtained from the general population , we aimed to investigate the effects of incentives and event rate on reaction time ( RT ) performance and response inhibition .
	manualset3
223857	6	420870	7	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Focusing on symptoms of attention deficit hyperactivity disorder ( ADHD ) in a sample obtained from the general population , we aimed to investigate the effects of incentives and event rate on reaction time ( RT ) performance and response inhibition .
	manualset3
223858	7	420870	7	NULL	NULL	0	NULL	incentives	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Focusing on symptoms of attention deficit hyperactivity disorder ( ADHD ) in a sample obtained from the general population , we aimed to investigate the effects of incentives and event rate on reaction time ( RT ) performance and response inhibition .
	manualset3
223859	8	420870	7	NULL	NULL	0	NULL	event rate 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Focusing on symptoms of attention deficit hyperactivity disorder ( ADHD ) in a sample obtained from the general population , we aimed to investigate the effects of incentives and event rate on reaction time ( RT ) performance and response inhibition .
	manualset3
223860	9	420870	7	NULL	NULL	0	NULL	reaction time ( RT ) performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Focusing on symptoms of attention deficit hyperactivity disorder ( ADHD ) in a sample obtained from the general population , we aimed to investigate the effects of incentives and event rate on reaction time ( RT ) performance and response inhibition .
	manualset3
223861	10	420870	7	NULL	NULL	0	NULL	response inhibition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Focusing on symptoms of attention deficit hyperactivity disorder ( ADHD ) in a sample obtained from the general population , we aimed to investigate the effects of incentives and event rate on reaction time ( RT ) performance and response inhibition .
	manualset3
223862	1	420871	7	NULL	NULL	0	NULL	 two models 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	They offer two models of valid consent : the objective model , which focuses on the congruence or lack of it between the patient and a `` reasonable '' person , and the subjective model , which focuses entirely on the patient 's actual understanding .
	manualset3
223863	2	420871	7	NULL	NULL	0	NULL	 valid consent	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They offer two models of valid consent : the objective model , which focuses on the congruence or lack of it between the patient and a `` reasonable '' person , and the subjective model , which focuses entirely on the patient 's actual understanding .
	manualset3
223864	3	420871	7	NULL	NULL	0	NULL	objective model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	They offer two models of valid consent : the objective model , which focuses on the congruence or lack of it between the patient and a `` reasonable '' person , and the subjective model , which focuses entirely on the patient 's actual understanding .
	manualset3
223865	4	420871	7	NULL	NULL	0	NULL	 congruence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They offer two models of valid consent : the objective model , which focuses on the congruence or lack of it between the patient and a `` reasonable '' person , and the subjective model , which focuses entirely on the patient 's actual understanding .
	manualset3
223866	5	420871	7	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	They offer two models of valid consent : the objective model , which focuses on the congruence or lack of it between the patient and a `` reasonable '' person , and the subjective model , which focuses entirely on the patient 's actual understanding .
	manualset3
223867	6	420871	7	NULL	NULL	0	NULL	`` reasonable '' person	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	They offer two models of valid consent : the objective model , which focuses on the congruence or lack of it between the patient and a `` reasonable '' person , and the subjective model , which focuses entirely on the patient 's actual understanding .
	manualset3
223868	7	420871	7	NULL	NULL	0	NULL	 subjective model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	They offer two models of valid consent : the objective model , which focuses on the congruence or lack of it between the patient and a `` reasonable '' person , and the subjective model , which focuses entirely on the patient 's actual understanding .
	manualset3
223869	8	420871	7	NULL	NULL	0	NULL	patient 's actual understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They offer two models of valid consent : the objective model , which focuses on the congruence or lack of it between the patient and a `` reasonable '' person , and the subjective model , which focuses entirely on the patient 's actual understanding .
	manualset3
223870	1	420872	7	NULL	NULL	0	NULL	Basal forebrain cholinergic cell attachment	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Basal forebrain cholinergic cell attachment and neurite outgrowth on organotypic slice cultures of hippocampal formation .
	manualset3
223871	2	420872	7	NULL	NULL	0	NULL	neurite outgrowth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Basal forebrain cholinergic cell attachment and neurite outgrowth on organotypic slice cultures of hippocampal formation .
	manualset3
223872	3	420872	7	NULL	NULL	0	NULL	organotypic slice cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Basal forebrain cholinergic cell attachment and neurite outgrowth on organotypic slice cultures of hippocampal formation .
	manualset3
223873	4	420872	7	NULL	NULL	0	NULL	hippocampal formation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Basal forebrain cholinergic cell attachment and neurite outgrowth on organotypic slice cultures of hippocampal formation .
	manualset3
223874	1	420873	7	NULL	NULL	0	NULL	Sequence 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence and functional properties of African green monkey CD4 silencer .
	manualset3
223875	2	420873	7	NULL	NULL	0	NULL	functional properties	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence and functional properties of African green monkey CD4 silencer .
	manualset3
223876	3	420873	7	NULL	NULL	0	NULL	African green monkey	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence and functional properties of African green monkey CD4 silencer .
	manualset3
223877	4	420873	7	NULL	NULL	0	NULL	CD4 silencer	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Sequence and functional properties of African green monkey CD4 silencer .
	manualset3
223878	1	420874	7	NULL	NULL	0	NULL	59 ( ( 18 ) F ) FDG-PET/CT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the 59 ( ( 18 ) F ) FDG-PET/CT , 29 were positive ( 26 had true-positive and 3 false-positive findings ) and 30 negative .
	manualset3
223879	2	420874	7	NULL	NULL	0	NULL	29	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the 59 ( ( 18 ) F ) FDG-PET/CT , 29 were positive ( 26 had true-positive and 3 false-positive findings ) and 30 negative .
	manualset3
223880	3	420874	7	NULL	NULL	0	NULL	positive	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the 59 ( ( 18 ) F ) FDG-PET/CT , 29 were positive ( 26 had true-positive and 3 false-positive findings ) and 30 negative .
	manualset3
223881	4	420874	7	NULL	NULL	0	NULL	26 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the 59 ( ( 18 ) F ) FDG-PET/CT , 29 were positive ( 26 had true-positive and 3 false-positive findings ) and 30 negative .
	manualset3
223882	5	420874	7	NULL	NULL	0	NULL	 true-positive findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the 59 ( ( 18 ) F ) FDG-PET/CT , 29 were positive ( 26 had true-positive and 3 false-positive findings ) and 30 negative .
	manualset3
223883	6	420874	7	NULL	NULL	0	NULL	3	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the 59 ( ( 18 ) F ) FDG-PET/CT , 29 were positive ( 26 had true-positive and 3 false-positive findings ) and 30 negative .
	manualset3
223884	7	420874	7	NULL	NULL	0	NULL	 false-positive findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the 59 ( ( 18 ) F ) FDG-PET/CT , 29 were positive ( 26 had true-positive and 3 false-positive findings ) and 30 negative .
	manualset3
223885	8	420874	7	NULL	NULL	0	NULL	 30	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the 59 ( ( 18 ) F ) FDG-PET/CT , 29 were positive ( 26 had true-positive and 3 false-positive findings ) and 30 negative .
	manualset3
223886	9	420874	7	NULL	NULL	0	NULL	negative	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the 59 ( ( 18 ) F ) FDG-PET/CT , 29 were positive ( 26 had true-positive and 3 false-positive findings ) and 30 negative .
	manualset3
223887	1	420875	7	NULL	NULL	0	NULL	Outcome 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Outcome and survival : Dutch experience with 110 patients studied prospectively .
	manualset3
223888	2	420875	7	NULL	NULL	NULL	NULL	survival	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	I. Outcome and survival : Dutch experience with 110 patients studied prospectively .
	manualset3
223889	3	420875	7	NULL	NULL	0	NULL	Dutch experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Outcome and survival : Dutch experience with 110 patients studied prospectively .
	manualset3
223890	4	420875	7	NULL	NULL	0	NULL	110 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Outcome and survival : Dutch experience with 110 patients studied prospectively .
	manualset3
223891	1	420876	7	NULL	NULL	0	NULL	SUA	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When a SUA is identified antenatally , a targeted ultrasound is warranted to rule out associated anomalies .
	manualset3
223892	2	420876	7	NULL	NULL	0	NULL	ultrasound 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	When a SUA is identified antenatally , a targeted ultrasound is warranted to rule out associated anomalies .
	manualset3
223893	3	420876	7	NULL	NULL	NULL	NULL	anomalies 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When a SUA is identified antenatally , a targeted ultrasound is warranted to rule out associated anomalies .
	manualset3
223894	1	420877	7	NULL	NULL	0	NULL	initial rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial rate was approximately 0.21 nmol of Ca2 + ( mg of protein ) -1 min-1 .
	manualset3
223895	2	420877	7	NULL	NULL	0	NULL	0.21 nmol 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial rate was approximately 0.21 nmol of Ca2 + ( mg of protein ) -1 min-1 .
	manualset3
223896	3	420877	7	NULL	NULL	0	NULL	Ca2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial rate was approximately 0.21 nmol of Ca2 + ( mg of protein ) -1 min-1 .
	manualset3
223897	4	420877	7	NULL	NULL	NULL	NULL	mg of protein -1 min-1	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The initial rate was approximately 0.21 nmol of Ca2 + ( mg of protein ) -1 min-1 .
	manualset3
223899	1	420878	7	NULL	NULL	0	NULL	average single-channel permeability coefficient 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average single-channel permeability coefficient of alpha-hemolysin for water ranged between 1.3x10-12 cm/s and 1.5x10-12 cm/s , depending on pH. .
	manualset3
223900	2	420878	7	NULL	NULL	0	NULL	alpha-hemolysin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The average single-channel permeability coefficient of alpha-hemolysin for water ranged between 1.3x10-12 cm/s and 1.5x10-12 cm/s , depending on pH. .
	manualset3
223901	3	420878	7	NULL	NULL	0	NULL	water 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The average single-channel permeability coefficient of alpha-hemolysin for water ranged between 1.3x10-12 cm/s and 1.5x10-12 cm/s , depending on pH. .
	manualset3
223902	4	420878	7	NULL	NULL	0	NULL	1.3x10-12 cm/s 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average single-channel permeability coefficient of alpha-hemolysin for water ranged between 1.3x10-12 cm/s and 1.5x10-12 cm/s , depending on pH. .
	manualset3
223903	5	420878	7	NULL	NULL	0	NULL	1.5x10-12 cm/s 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average single-channel permeability coefficient of alpha-hemolysin for water ranged between 1.3x10-12 cm/s and 1.5x10-12 cm/s , depending on pH. .
	manualset3
223904	6	420878	7	NULL	NULL	0	NULL	pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The average single-channel permeability coefficient of alpha-hemolysin for water ranged between 1.3x10-12 cm/s and 1.5x10-12 cm/s , depending on pH. .
	manualset3
223905	1	420879	7	NULL	NULL	0	NULL	Reduced stride length	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced stride length characterizes Parkinsonian gait .
	manualset3
223906	2	420879	7	NULL	NULL	0	NULL	Parkinsonian gait	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Reduced stride length characterizes Parkinsonian gait .
	manualset3
223907	1	420880	7	NULL	NULL	0	NULL	MMP activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MMP activities were determined by SDS-gelatin - , casein - , and carboxymethyl transferrin-polyacrylamide gel zymography .
	manualset3
223908	2	420880	7	NULL	NULL	NULL	NULL	SDS-gelatin - polyacrylamide gel zymography	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	MMP activities were determined by SDS-gelatin - , casein - , and carboxymethyl transferrin-polyacrylamide gel zymography .
	manualset3
223909	3	420880	7	NULL	NULL	0	NULL	casein - polyacrylamide gel zymography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	MMP activities were determined by SDS-gelatin - , casein - , and carboxymethyl transferrin-polyacrylamide gel zymography .
	manualset3
223910	4	420880	7	NULL	NULL	0	NULL	carboxymethyl transferrin-polyacrylamide gel zymography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	MMP activities were determined by SDS-gelatin - , casein - , and carboxymethyl transferrin-polyacrylamide gel zymography .
	manualset3
223911	1	420881	7	NULL	NULL	0	NULL	higher depression scores	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The higher depression scores in gastric ulcer patients , however , simply reflected the greater chronicity of their physical symptoms .
	manualset3
223912	2	420881	7	NULL	NULL	0	NULL	gastric ulcer patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The higher depression scores in gastric ulcer patients , however , simply reflected the greater chronicity of their physical symptoms .
	manualset3
223913	3	420881	7	NULL	NULL	0	NULL	greater chronicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The higher depression scores in gastric ulcer patients , however , simply reflected the greater chronicity of their physical symptoms .
	manualset3
223914	4	420881	7	NULL	NULL	0	NULL	physical symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The higher depression scores in gastric ulcer patients , however , simply reflected the greater chronicity of their physical symptoms .
	manualset3
225380	1	420882	7	NULL	NULL	0	NULL	follow-up	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Those lost to follow-up were more ` socially stable ' on initial measures than those successfully contacted .
	manualset3
225381	2	420882	7	NULL	NULL	0	NULL	 socially stable	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Those lost to follow-up were more ` socially stable ' on initial measures than those successfully contacted .
	manualset3
225382	3	420882	7	NULL	NULL	0	NULL	initial measures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Those lost to follow-up were more ` socially stable ' on initial measures than those successfully contacted .
	manualset3
225383	1	420883	7	NULL	NULL	0	NULL	 acoustic method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	An acoustic method has long been proposed for cavitation detection .
	manualset3
225384	2	420883	7	NULL	NULL	0	NULL	cavitation detection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An acoustic method has long been proposed for cavitation detection .
	manualset3
223915	1	420884	7	NULL	NULL	0	NULL	T-20	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	AtT-20 , was able to efficiently cleave pro-enkephalin to smaller peptides including Met-enkephalin .
	manualset3
223916	2	420884	7	NULL	NULL	0	NULL	pro-enkephalin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	AtT-20 , was able to efficiently cleave pro-enkephalin to smaller peptides including Met-enkephalin .
	manualset3
223917	3	420884	7	NULL	NULL	0	NULL	smaller peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	AtT-20 , was able to efficiently cleave pro-enkephalin to smaller peptides including Met-enkephalin .
	manualset3
223918	4	420884	7	NULL	NULL	0	NULL	Met-enkephalin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	AtT-20 , was able to efficiently cleave pro-enkephalin to smaller peptides including Met-enkephalin .
	manualset3
223919	1	420885	7	NULL	NULL	0	NULL	Fever 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Fever of unknown origin due to primary mycotic aneurysm of the aorta ) .
	manualset3
223920	2	420885	7	NULL	NULL	0	NULL	unknown origin 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Fever of unknown origin due to primary mycotic aneurysm of the aorta ) .
	manualset3
223921	3	420885	7	NULL	NULL	0	NULL	primary mycotic aneurysm	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Fever of unknown origin due to primary mycotic aneurysm of the aorta ) .
	manualset3
223922	4	420885	7	NULL	NULL	0	NULL	aorta 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Fever of unknown origin due to primary mycotic aneurysm of the aorta ) .
	manualset3
223923	1	420886	7	NULL	NULL	0	NULL	structure-activity relationship study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure-activity relationship study revealed that substituents including 3 , 4 , 5-trimethoxyphenyl , 3 , 4-dimethoxyphenyl , 4-benzyloxy-3-methoxyphenyl , 4-piperidinyl , 4-fluorophenyl and N-methylindole are beneficial for the activity of indolyl-1 , 2 , 4 - triazoles ( 6 and 7 ) .
	manualset3
223924	2	420886	7	NULL	NULL	0	NULL	 substituents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure-activity relationship study revealed that substituents including 3 , 4 , 5-trimethoxyphenyl , 3 , 4-dimethoxyphenyl , 4-benzyloxy-3-methoxyphenyl , 4-piperidinyl , 4-fluorophenyl and N-methylindole are beneficial for the activity of indolyl-1 , 2 , 4 - triazoles ( 6 and 7 ) .
	manualset3
223925	3	420886	7	NULL	NULL	0	NULL	3 , 4 , 5-trimethoxyphenyl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure-activity relationship study revealed that substituents including 3 , 4 , 5-trimethoxyphenyl , 3 , 4-dimethoxyphenyl , 4-benzyloxy-3-methoxyphenyl , 4-piperidinyl , 4-fluorophenyl and N-methylindole are beneficial for the activity of indolyl-1 , 2 , 4 - triazoles ( 6 and 7 ) .
	manualset3
223926	4	420886	7	NULL	NULL	0	NULL	3 , 4-dimethoxyphenyl 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure-activity relationship study revealed that substituents including 3 , 4 , 5-trimethoxyphenyl , 3 , 4-dimethoxyphenyl , 4-benzyloxy-3-methoxyphenyl , 4-piperidinyl , 4-fluorophenyl and N-methylindole are beneficial for the activity of indolyl-1 , 2 , 4 - triazoles ( 6 and 7 ) .
	manualset3
223927	5	420886	7	NULL	NULL	0	NULL	4-benzyloxy-3-methoxyphenyl 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure-activity relationship study revealed that substituents including 3 , 4 , 5-trimethoxyphenyl , 3 , 4-dimethoxyphenyl , 4-benzyloxy-3-methoxyphenyl , 4-piperidinyl , 4-fluorophenyl and N-methylindole are beneficial for the activity of indolyl-1 , 2 , 4 - triazoles ( 6 and 7 ) .
	manualset3
223928	6	420886	7	NULL	NULL	0	NULL	4-piperidinyl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure-activity relationship study revealed that substituents including 3 , 4 , 5-trimethoxyphenyl , 3 , 4-dimethoxyphenyl , 4-benzyloxy-3-methoxyphenyl , 4-piperidinyl , 4-fluorophenyl and N-methylindole are beneficial for the activity of indolyl-1 , 2 , 4 - triazoles ( 6 and 7 ) .
	manualset3
223929	7	420886	7	NULL	NULL	0	NULL	4-fluorophenyl 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure-activity relationship study revealed that substituents including 3 , 4 , 5-trimethoxyphenyl , 3 , 4-dimethoxyphenyl , 4-benzyloxy-3-methoxyphenyl , 4-piperidinyl , 4-fluorophenyl and N-methylindole are beneficial for the activity of indolyl-1 , 2 , 4 - triazoles ( 6 and 7 ) .
	manualset3
223930	8	420886	7	NULL	NULL	0	NULL	N-methylindole	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure-activity relationship study revealed that substituents including 3 , 4 , 5-trimethoxyphenyl , 3 , 4-dimethoxyphenyl , 4-benzyloxy-3-methoxyphenyl , 4-piperidinyl , 4-fluorophenyl and N-methylindole are beneficial for the activity of indolyl-1 , 2 , 4 - triazoles ( 6 and 7 ) .
	manualset3
223931	9	420886	7	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The structure-activity relationship study revealed that substituents including 3 , 4 , 5-trimethoxyphenyl , 3 , 4-dimethoxyphenyl , 4-benzyloxy-3-methoxyphenyl , 4-piperidinyl , 4-fluorophenyl and N-methylindole are beneficial for the activity of indolyl-1 , 2 , 4 - triazoles ( 6 and 7 ) .
	manualset3
223932	10	420886	7	NULL	NULL	NULL	NULL	indolyl-1 , 2 , 4 - triazoles ( 6 and 7 )  	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The structure-activity relationship study revealed that substituents including 3 , 4 , 5-trimethoxyphenyl , 3 , 4-dimethoxyphenyl , 4-benzyloxy-3-methoxyphenyl , 4-piperidinyl , 4-fluorophenyl and N-methylindole are beneficial for the activity of indolyl-1 , 2 , 4 - triazoles ( 6 and 7 ) .
	manualset3
223933	1	420887	7	NULL	NULL	0	NULL	Src64B overexpression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Though Src64B overexpression induced the formation of specialized hemocytes known as lamellocytes , its hyperactivation had no effect on circulating plasmatocyte concentration .
	manualset3
223934	2	420887	7	NULL	NULL	0	NULL	formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Though Src64B overexpression induced the formation of specialized hemocytes known as lamellocytes , its hyperactivation had no effect on circulating plasmatocyte concentration .
	manualset3
223935	3	420887	7	NULL	NULL	0	NULL	specialized hemocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Though Src64B overexpression induced the formation of specialized hemocytes known as lamellocytes , its hyperactivation had no effect on circulating plasmatocyte concentration .
	manualset3
223936	4	420887	7	NULL	NULL	0	NULL	 lamellocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Though Src64B overexpression induced the formation of specialized hemocytes known as lamellocytes , its hyperactivation had no effect on circulating plasmatocyte concentration .
	manualset3
223937	5	420887	7	NULL	NULL	0	NULL	hyperactivation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Though Src64B overexpression induced the formation of specialized hemocytes known as lamellocytes , its hyperactivation had no effect on circulating plasmatocyte concentration .
	manualset3
223938	6	420887	7	NULL	NULL	NULL	NULL	no effect 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Though Src64B overexpression induced the formation of specialized hemocytes known as lamellocytes , its hyperactivation had no effect on circulating plasmatocyte concentration .
	manualset3
223939	7	420887	7	NULL	NULL	0	NULL	circulating plasmatocyte concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Though Src64B overexpression induced the formation of specialized hemocytes known as lamellocytes , its hyperactivation had no effect on circulating plasmatocyte concentration .
	manualset3
223940	1	420888	7	NULL	NULL	0	NULL	Detecton	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Detecton of circulating antigen in sera from mice infected with Toxoplasma tachyzoites ) .
	manualset3
223941	2	420888	7	NULL	NULL	0	NULL	circulating antigen	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Detecton of circulating antigen in sera from mice infected with Toxoplasma tachyzoites ) .
	manualset3
223942	3	420888	7	NULL	NULL	0	NULL	sera	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Detecton of circulating antigen in sera from mice infected with Toxoplasma tachyzoites ) .
	manualset3
223943	4	420888	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Detecton of circulating antigen in sera from mice infected with Toxoplasma tachyzoites ) .
	manualset3
223944	5	420888	7	NULL	NULL	0	NULL	Toxoplasma tachyzoites	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Detecton of circulating antigen in sera from mice infected with Toxoplasma tachyzoites ) .
	manualset3
223945	1	420889	7	NULL	NULL	0	NULL	V. cholerae 01 strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the V. cholerae 01 strains isolated after July 1993 , 4 PFGE banding designated as H through K were observed with pattern H dominating .
	manualset3
223946	2	420889	7	NULL	NULL	0	NULL	July 1993	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the V. cholerae 01 strains isolated after July 1993 , 4 PFGE banding designated as H through K were observed with pattern H dominating .
	manualset3
223947	3	420889	7	NULL	NULL	0	NULL	4 PFGE banding 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the V. cholerae 01 strains isolated after July 1993 , 4 PFGE banding designated as H through K were observed with pattern H dominating .
	manualset3
223948	4	420889	7	NULL	NULL	0	NULL	 H through K	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the V. cholerae 01 strains isolated after July 1993 , 4 PFGE banding designated as H through K were observed with pattern H dominating .
	manualset3
223949	5	420889	7	NULL	NULL	0	NULL	 pattern H dominating	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the V. cholerae 01 strains isolated after July 1993 , 4 PFGE banding designated as H through K were observed with pattern H dominating .
	manualset3
223950	1	420890	7	NULL	NULL	0	NULL	5-Fluorouracil infusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	5-Fluorouracil infusion and alpha interferon is a potentially useful combination that needs further evaluation in future phase II and phase III trials .
	manualset3
223951	2	420890	7	NULL	NULL	0	NULL	alpha interferon	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	5-Fluorouracil infusion and alpha interferon is a potentially useful combination that needs further evaluation in future phase II and phase III trials .
	manualset3
223952	3	420890	7	NULL	NULL	0	NULL	combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	5-Fluorouracil infusion and alpha interferon is a potentially useful combination that needs further evaluation in future phase II and phase III trials .
	manualset3
223953	4	420890	7	NULL	NULL	0	NULL	evaluation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	5-Fluorouracil infusion and alpha interferon is a potentially useful combination that needs further evaluation in future phase II and phase III trials .
	manualset3
223954	5	420890	7	NULL	NULL	0	NULL	future phase II trials	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	5-Fluorouracil infusion and alpha interferon is a potentially useful combination that needs further evaluation in future phase II and phase III trials .
	manualset3
223955	6	420890	7	NULL	NULL	0	NULL	phase III trials 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	5-Fluorouracil infusion and alpha interferon is a potentially useful combination that needs further evaluation in future phase II and phase III trials .
	manualset3
223956	1	420891	7	NULL	NULL	0	NULL	President 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	President names members of peace institute .
	manualset3
223957	2	420891	7	NULL	NULL	0	NULL	members	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	President names members of peace institute .
	manualset3
223958	3	420891	7	NULL	NULL	0	NULL	peace institute 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	President names members of peace institute .
	manualset3
223959	1	420892	7	NULL	NULL	0	NULL	 identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of these enzymes was possible by MICs determination against a set of aminoglycosides antibiotics .
	manualset3
223960	2	420892	7	NULL	NULL	0	NULL	enzymes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of these enzymes was possible by MICs determination against a set of aminoglycosides antibiotics .
	manualset3
223961	3	420892	7	NULL	NULL	0	NULL	MICs determination 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of these enzymes was possible by MICs determination against a set of aminoglycosides antibiotics .
	manualset3
223962	4	420892	7	NULL	NULL	0	NULL	set	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of these enzymes was possible by MICs determination against a set of aminoglycosides antibiotics .
	manualset3
223963	5	420892	7	NULL	NULL	0	NULL	 aminoglycosides antibiotics 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The identification of these enzymes was possible by MICs determination against a set of aminoglycosides antibiotics .
	manualset3
223964	1	420893	7	NULL	NULL	0	NULL	excision	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After excision of a section of tissue from the plantar aspect of the digit and partial section of the deep digital flexor tendon , the distal sesamoid bone was excised .
	manualset3
223965	2	420893	7	NULL	NULL	0	NULL	section of tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	After excision of a section of tissue from the plantar aspect of the digit and partial section of the deep digital flexor tendon , the distal sesamoid bone was excised .
	manualset3
223966	3	420893	7	NULL	NULL	0	NULL	plantar aspect of the digit	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After excision of a section of tissue from the plantar aspect of the digit and partial section of the deep digital flexor tendon , the distal sesamoid bone was excised .
	manualset3
223967	4	420893	7	NULL	NULL	0	NULL	partial section	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After excision of a section of tissue from the plantar aspect of the digit and partial section of the deep digital flexor tendon , the distal sesamoid bone was excised .
	manualset3
223968	5	420893	7	NULL	NULL	0	NULL	deep digital flexor tendon	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After excision of a section of tissue from the plantar aspect of the digit and partial section of the deep digital flexor tendon , the distal sesamoid bone was excised .
	manualset3
223969	6	420893	7	NULL	NULL	0	NULL	distal sesamoid bone	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	After excision of a section of tissue from the plantar aspect of the digit and partial section of the deep digital flexor tendon , the distal sesamoid bone was excised .
	manualset3
223970	1	420894	7	NULL	NULL	0	NULL	Expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of the human telomerase catalytic subunit restored the telomerase activity in the sheep cells and extended their proliferative life span .
	manualset3
223971	2	420894	7	NULL	NULL	0	NULL	human telomerase catalytic subunit	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of the human telomerase catalytic subunit restored the telomerase activity in the sheep cells and extended their proliferative life span .
	manualset3
223972	3	420894	7	NULL	NULL	0	NULL	telomerase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of the human telomerase catalytic subunit restored the telomerase activity in the sheep cells and extended their proliferative life span .
	manualset3
223973	4	420894	7	NULL	NULL	0	NULL	sheep cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of the human telomerase catalytic subunit restored the telomerase activity in the sheep cells and extended their proliferative life span .
	manualset3
223974	5	420894	7	NULL	NULL	0	NULL	proliferative life span 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of the human telomerase catalytic subunit restored the telomerase activity in the sheep cells and extended their proliferative life span .
	manualset3
223975	1	420895	7	NULL	NULL	0	NULL	Kinetic analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Kinetic analyses of the reaction revealed that a dimer caused by intermolecular interaction of 2S rRNA may be the substrate for the cleavage between 11 and 12 , while a simple monomer is the substrate for the cleavage between 16 and 17 .
	manualset3
223976	2	420895	7	NULL	NULL	0	NULL	reaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Kinetic analyses of the reaction revealed that a dimer caused by intermolecular interaction of 2S rRNA may be the substrate for the cleavage between 11 and 12 , while a simple monomer is the substrate for the cleavage between 16 and 17 .
	manualset3
223977	3	420895	7	NULL	NULL	0	NULL	dimer	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Kinetic analyses of the reaction revealed that a dimer caused by intermolecular interaction of 2S rRNA may be the substrate for the cleavage between 11 and 12 , while a simple monomer is the substrate for the cleavage between 16 and 17 .
	manualset3
223978	4	420895	7	NULL	NULL	0	NULL	intermolecular interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Kinetic analyses of the reaction revealed that a dimer caused by intermolecular interaction of 2S rRNA may be the substrate for the cleavage between 11 and 12 , while a simple monomer is the substrate for the cleavage between 16 and 17 .
	manualset3
223979	5	420895	7	NULL	NULL	0	NULL	 2S rRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Kinetic analyses of the reaction revealed that a dimer caused by intermolecular interaction of 2S rRNA may be the substrate for the cleavage between 11 and 12 , while a simple monomer is the substrate for the cleavage between 16 and 17 .
	manualset3
223980	6	420895	7	NULL	NULL	0	NULL	substrate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Kinetic analyses of the reaction revealed that a dimer caused by intermolecular interaction of 2S rRNA may be the substrate for the cleavage between 11 and 12 , while a simple monomer is the substrate for the cleavage between 16 and 17 .
	manualset3
223981	7	420895	7	NULL	NULL	0	NULL	cleavage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Kinetic analyses of the reaction revealed that a dimer caused by intermolecular interaction of 2S rRNA may be the substrate for the cleavage between 11 and 12 , while a simple monomer is the substrate for the cleavage between 16 and 17 .
	manualset3
223982	8	420895	7	NULL	NULL	NULL	NULL	 11 and 12	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Kinetic analyses of the reaction revealed that a dimer caused by intermolecular interaction of 2S rRNA may be the substrate for the cleavage between 11 and 12 , while a simple monomer is the substrate for the cleavage between 16 and 17 .
	manualset3
223983	9	420895	7	NULL	NULL	0	NULL	simple monomer	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Kinetic analyses of the reaction revealed that a dimer caused by intermolecular interaction of 2S rRNA may be the substrate for the cleavage between 11 and 12 , while a simple monomer is the substrate for the cleavage between 16 and 17 .
	manualset3
223984	10	420895	7	NULL	NULL	0	NULL	substrate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Kinetic analyses of the reaction revealed that a dimer caused by intermolecular interaction of 2S rRNA may be the substrate for the cleavage between 11 and 12 , while a simple monomer is the substrate for the cleavage between 16 and 17 .
	manualset3
223985	11	420895	7	NULL	NULL	0	NULL	cleavage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Kinetic analyses of the reaction revealed that a dimer caused by intermolecular interaction of 2S rRNA may be the substrate for the cleavage between 11 and 12 , while a simple monomer is the substrate for the cleavage between 16 and 17 .
	manualset3
223986	12	420895	7	NULL	NULL	0	NULL	16 and 17 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Kinetic analyses of the reaction revealed that a dimer caused by intermolecular interaction of 2S rRNA may be the substrate for the cleavage between 11 and 12 , while a simple monomer is the substrate for the cleavage between 16 and 17 .
	manualset3
223987	1	420896	7	NULL	NULL	0	NULL	apparatus	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The apparatus is diffraction limited at f/31 .4 .
	manualset3
223988	2	420896	7	NULL	NULL	0	NULL	 diffraction limited	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The apparatus is diffraction limited at f/31 .4 .
	manualset3
223989	3	420896	7	NULL	NULL	0	NULL	f/31 .4	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The apparatus is diffraction limited at f/31 .4 .
	manualset3
223990	1	420897	7	NULL	NULL	0	NULL	High Na + concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	High Na + concentrations preferentially maintain the E1 conformation of the enzyme , which is less stable against denaturation during the dialysis , but displays a higher percentage of inside-out orientation of the transport-active protein .
	manualset3
223991	2	420897	7	NULL	NULL	0	NULL	E1 conformation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	High Na + concentrations preferentially maintain the E1 conformation of the enzyme , which is less stable against denaturation during the dialysis , but displays a higher percentage of inside-out orientation of the transport-active protein .
	manualset3
223992	3	420897	7	NULL	NULL	0	NULL	enzyme	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	High Na + concentrations preferentially maintain the E1 conformation of the enzyme , which is less stable against denaturation during the dialysis , but displays a higher percentage of inside-out orientation of the transport-active protein .
	manualset3
223993	4	420897	7	NULL	NULL	0	NULL	denaturation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	High Na + concentrations preferentially maintain the E1 conformation of the enzyme , which is less stable against denaturation during the dialysis , but displays a higher percentage of inside-out orientation of the transport-active protein .
	manualset3
223994	5	420897	7	NULL	NULL	0	NULL	dialysis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	High Na + concentrations preferentially maintain the E1 conformation of the enzyme , which is less stable against denaturation during the dialysis , but displays a higher percentage of inside-out orientation of the transport-active protein .
	manualset3
223995	6	420897	7	NULL	NULL	0	NULL	higher percentage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	High Na + concentrations preferentially maintain the E1 conformation of the enzyme , which is less stable against denaturation during the dialysis , but displays a higher percentage of inside-out orientation of the transport-active protein .
	manualset3
223996	7	420897	7	NULL	NULL	0	NULL	inside-out orientation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	High Na + concentrations preferentially maintain the E1 conformation of the enzyme , which is less stable against denaturation during the dialysis , but displays a higher percentage of inside-out orientation of the transport-active protein .
	manualset3
223997	8	420897	7	NULL	NULL	0	NULL	transport-active protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	High Na + concentrations preferentially maintain the E1 conformation of the enzyme , which is less stable against denaturation during the dialysis , but displays a higher percentage of inside-out orientation of the transport-active protein .
	manualset3
223998	1	420898	7	NULL	NULL	0	NULL	advantages 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the advantages of such a test are that the patient does not receive ionizing radiation ; it is independent of the presence of iodide-or mercury-containing compounds ; and it minimizes the number of patient visits .
	manualset3
223999	2	420898	7	NULL	NULL	0	NULL	test 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the advantages of such a test are that the patient does not receive ionizing radiation ; it is independent of the presence of iodide-or mercury-containing compounds ; and it minimizes the number of patient visits .
	manualset3
224000	3	420898	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the advantages of such a test are that the patient does not receive ionizing radiation ; it is independent of the presence of iodide-or mercury-containing compounds ; and it minimizes the number of patient visits .
	manualset3
224001	4	420898	7	NULL	NULL	NULL	NULL	ionizing radiation	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Among the advantages of such a test are that the patient does not receive ionizing radiation ; it is independent of the presence of iodide-or mercury-containing compounds ; and it minimizes the number of patient visits .
	manualset3
224002	5	420898	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the advantages of such a test are that the patient does not receive ionizing radiation ; it is independent of the presence of iodide-or mercury-containing compounds ; and it minimizes the number of patient visits .
	manualset3
224003	6	420898	7	NULL	NULL	0	NULL	iodide-or mercury-containing compounds 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the advantages of such a test are that the patient does not receive ionizing radiation ; it is independent of the presence of iodide-or mercury-containing compounds ; and it minimizes the number of patient visits .
	manualset3
224004	7	420898	7	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the advantages of such a test are that the patient does not receive ionizing radiation ; it is independent of the presence of iodide-or mercury-containing compounds ; and it minimizes the number of patient visits .
	manualset3
224005	8	420898	7	NULL	NULL	0	NULL	 patient visits	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the advantages of such a test are that the patient does not receive ionizing radiation ; it is independent of the presence of iodide-or mercury-containing compounds ; and it minimizes the number of patient visits .
	manualset3
224006	1	420899	7	NULL	NULL	0	NULL	telomere shortening	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	How telomere shortening triggers cell senescence and whether it contributes to aging in vivo are under investigation .
	manualset3
224007	2	420899	7	NULL	NULL	0	NULL	cell senescence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	How telomere shortening triggers cell senescence and whether it contributes to aging in vivo are under investigation .
	manualset3
224008	3	420899	7	NULL	NULL	0	NULL	aging	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	How telomere shortening triggers cell senescence and whether it contributes to aging in vivo are under investigation .
	manualset3
224009	4	420899	7	NULL	NULL	0	NULL	investigation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	How telomere shortening triggers cell senescence and whether it contributes to aging in vivo are under investigation .
	manualset3
224010	1	420900	7	NULL	NULL	0	NULL	thyroid stimulating hormone 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Persistently raised thyroid stimulating hormone in adequately treated congenital hypothyroidism on long-term follow-up .
	manualset3
224011	2	420900	7	NULL	NULL	0	NULL	 congenital hypothyroidism	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Persistently raised thyroid stimulating hormone in adequately treated congenital hypothyroidism on long-term follow-up .
	manualset3
224012	3	420900	7	NULL	NULL	0	NULL	long-term follow-up	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Persistently raised thyroid stimulating hormone in adequately treated congenital hypothyroidism on long-term follow-up .
	manualset3
224013	1	420901	7	NULL	NULL	0	NULL	Pregnancy rates	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnancy rates with endometriosis-associated infertility may be improved by laparoscopic surgery or laparotomy for moderate to severe disease .
	manualset3
224014	2	420901	7	NULL	NULL	NULL	NULL	endometriosis-associated infertility	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pregnancy rates with endometriosis-associated infertility may be improved by laparoscopic surgery or laparotomy for moderate to severe disease .
	manualset3
224015	3	420901	7	NULL	NULL	0	NULL	laparoscopic surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnancy rates with endometriosis-associated infertility may be improved by laparoscopic surgery or laparotomy for moderate to severe disease .
	manualset3
224016	4	420901	7	NULL	NULL	0	NULL	laparotomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnancy rates with endometriosis-associated infertility may be improved by laparoscopic surgery or laparotomy for moderate to severe disease .
	manualset3
224017	5	420901	7	NULL	NULL	0	NULL	moderate disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnancy rates with endometriosis-associated infertility may be improved by laparoscopic surgery or laparotomy for moderate to severe disease .
	manualset3
224018	6	420901	7	NULL	NULL	0	NULL	severe disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pregnancy rates with endometriosis-associated infertility may be improved by laparoscopic surgery or laparotomy for moderate to severe disease .
	manualset3
224019	1	420902	7	NULL	NULL	0	NULL	RT-PCR technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This RT-PCR technique was performed on sectioned tissues of female buds of the cucumber GY3 inbred line .
	manualset3
224020	2	420902	7	NULL	NULL	0	NULL	sectioned tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	This RT-PCR technique was performed on sectioned tissues of female buds of the cucumber GY3 inbred line .
	manualset3
224021	3	420902	7	NULL	NULL	0	NULL	female buds	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This RT-PCR technique was performed on sectioned tissues of female buds of the cucumber GY3 inbred line .
	manualset3
224022	4	420902	7	NULL	NULL	0	NULL	 cucumber GY3 inbred line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	This RT-PCR technique was performed on sectioned tissues of female buds of the cucumber GY3 inbred line .
	manualset3
224023	1	420903	7	NULL	NULL	0	NULL	Failure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Failure of single dose amoxycillin as prophylaxis against endocarditis .
	manualset3
224024	2	420903	7	NULL	NULL	0	NULL	 single dose 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Failure of single dose amoxycillin as prophylaxis against endocarditis .
	manualset3
224025	3	420903	7	NULL	NULL	0	NULL	amoxycillin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Failure of single dose amoxycillin as prophylaxis against endocarditis .
	manualset3
224026	4	420903	7	NULL	NULL	0	NULL	prophylaxis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Failure of single dose amoxycillin as prophylaxis against endocarditis .
	manualset3
224027	5	420903	7	NULL	NULL	0	NULL	endocarditis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Failure of single dose amoxycillin as prophylaxis against endocarditis .
	manualset3
224028	1	420904	7	NULL	NULL	0	NULL	Current concepts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Current concepts of oxygen-transporting blood substitutes .
	manualset3
224029	2	420904	7	NULL	NULL	0	NULL	oxygen-transporting blood substitutes	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Current concepts of oxygen-transporting blood substitutes .
	manualset3
224030	1	420905	7	NULL	NULL	0	NULL	clinical study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A clinical study from the viewpoint of differentiation from schizophrenia ) .
	manualset3
224031	2	420905	7	NULL	NULL	0	NULL	viewpoint	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A clinical study from the viewpoint of differentiation from schizophrenia ) .
	manualset3
224032	3	420905	7	NULL	NULL	0	NULL	differentiation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A clinical study from the viewpoint of differentiation from schizophrenia ) .
	manualset3
224033	4	420905	7	NULL	NULL	0	NULL	schizophrenia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A clinical study from the viewpoint of differentiation from schizophrenia ) .
	manualset3
224034	1	420906	7	NULL	NULL	0	NULL	Isometric lifting strength	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isometric and dynamic lifting strength , body composition and maximal box-lift to 1.45 m and 1.70 m were assessed before and after training .
	manualset3
224035	2	420906	7	NULL	NULL	0	NULL	dynamic lifting strength	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isometric and dynamic lifting strength , body composition and maximal box-lift to 1.45 m and 1.70 m were assessed before and after training .
	manualset3
224036	3	420906	7	NULL	NULL	0	NULL	body composition	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isometric and dynamic lifting strength , body composition and maximal box-lift to 1.45 m and 1.70 m were assessed before and after training .
	manualset3
224037	4	420906	7	NULL	NULL	0	NULL	maximal box-lift	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Isometric and dynamic lifting strength , body composition and maximal box-lift to 1.45 m and 1.70 m were assessed before and after training .
	manualset3
224038	5	420906	7	NULL	NULL	0	NULL	 1.45 m	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isometric and dynamic lifting strength , body composition and maximal box-lift to 1.45 m and 1.70 m were assessed before and after training .
	manualset3
224039	6	420906	7	NULL	NULL	0	NULL	1.70 m	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isometric and dynamic lifting strength , body composition and maximal box-lift to 1.45 m and 1.70 m were assessed before and after training .
	manualset3
224040	7	420906	7	NULL	NULL	0	NULL	training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Isometric and dynamic lifting strength , body composition and maximal box-lift to 1.45 m and 1.70 m were assessed before and after training .
	manualset3
224041	1	420907	7	NULL	NULL	0	NULL	limits of detection ( LOD )	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The limits of detection ( LOD ) and quantification ( LOQ ) of tungsten ( VI ) were found 7.51 and 24.75 gL ( -1 ) , respectively .
	manualset3
224042	2	420907	7	NULL	NULL	0	NULL	quantification ( LOQ ) of tungsten ( VI )	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The limits of detection ( LOD ) and quantification ( LOQ ) of tungsten ( VI ) were found 7.51 and 24.75 gL ( -1 ) , respectively .
	manualset3
224043	3	420907	7	NULL	NULL	0	NULL	7.51	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The limits of detection ( LOD ) and quantification ( LOQ ) of tungsten ( VI ) were found 7.51 and 24.75 gL ( -1 ) , respectively .
	manualset3
224044	4	420907	7	NULL	NULL	0	NULL	 24.75 gL ( -1 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The limits of detection ( LOD ) and quantification ( LOQ ) of tungsten ( VI ) were found 7.51 and 24.75 gL ( -1 ) , respectively .
	manualset3
224045	1	420908	7	NULL	NULL	0	NULL	 apoA-I-containing lipoproteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the apoA-I-containing lipoproteins isolated by selected-affinity immunosorption from human serum and plasma , we have identified a subpopulation which , unlike the bulk of high density lipoproteins , has pre-beta electrophoretic mobility .
	manualset3
224046	2	420908	7	NULL	NULL	0	NULL	selected-affinity immunosorption	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the apoA-I-containing lipoproteins isolated by selected-affinity immunosorption from human serum and plasma , we have identified a subpopulation which , unlike the bulk of high density lipoproteins , has pre-beta electrophoretic mobility .
	manualset3
224047	3	420908	7	NULL	NULL	0	NULL	human serum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the apoA-I-containing lipoproteins isolated by selected-affinity immunosorption from human serum and plasma , we have identified a subpopulation which , unlike the bulk of high density lipoproteins , has pre-beta electrophoretic mobility .
	manualset3
224048	4	420908	7	NULL	NULL	0	NULL	plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the apoA-I-containing lipoproteins isolated by selected-affinity immunosorption from human serum and plasma , we have identified a subpopulation which , unlike the bulk of high density lipoproteins , has pre-beta electrophoretic mobility .
	manualset3
224049	5	420908	7	NULL	NULL	0	NULL	subpopulation 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the apoA-I-containing lipoproteins isolated by selected-affinity immunosorption from human serum and plasma , we have identified a subpopulation which , unlike the bulk of high density lipoproteins , has pre-beta electrophoretic mobility .
	manualset3
224050	6	420908	7	NULL	NULL	0	NULL	 bulk 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the apoA-I-containing lipoproteins isolated by selected-affinity immunosorption from human serum and plasma , we have identified a subpopulation which , unlike the bulk of high density lipoproteins , has pre-beta electrophoretic mobility .
	manualset3
224051	7	420908	7	NULL	NULL	0	NULL	high density lipoproteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the apoA-I-containing lipoproteins isolated by selected-affinity immunosorption from human serum and plasma , we have identified a subpopulation which , unlike the bulk of high density lipoproteins , has pre-beta electrophoretic mobility .
	manualset3
224052	8	420908	7	NULL	NULL	0	NULL	pre-beta electrophoretic mobility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the apoA-I-containing lipoproteins isolated by selected-affinity immunosorption from human serum and plasma , we have identified a subpopulation which , unlike the bulk of high density lipoproteins , has pre-beta electrophoretic mobility .
	manualset3
224053	1	420909	7	NULL	NULL	0	NULL	female reproductive pattern	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The female reproductive pattern of the killer whale is characterized by a gestation of 17 mo and an ovarian cycle of 6-7 wk in duration .
	manualset3
224054	2	420909	7	NULL	NULL	0	NULL	killer whale 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The female reproductive pattern of the killer whale is characterized by a gestation of 17 mo and an ovarian cycle of 6-7 wk in duration .
	manualset3
224055	3	420909	7	NULL	NULL	0	NULL	gestation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The female reproductive pattern of the killer whale is characterized by a gestation of 17 mo and an ovarian cycle of 6-7 wk in duration .
	manualset3
224056	4	420909	7	NULL	NULL	0	NULL	17 mo 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The female reproductive pattern of the killer whale is characterized by a gestation of 17 mo and an ovarian cycle of 6-7 wk in duration .
	manualset3
224057	5	420909	7	NULL	NULL	0	NULL	ovarian cycle	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The female reproductive pattern of the killer whale is characterized by a gestation of 17 mo and an ovarian cycle of 6-7 wk in duration .
	manualset3
224058	6	420909	7	NULL	NULL	0	NULL	6-7 wk	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The female reproductive pattern of the killer whale is characterized by a gestation of 17 mo and an ovarian cycle of 6-7 wk in duration .
	manualset3
224059	7	420909	7	NULL	NULL	0	NULL	 duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The female reproductive pattern of the killer whale is characterized by a gestation of 17 mo and an ovarian cycle of 6-7 wk in duration .
	manualset3
224060	1	420910	7	NULL	NULL	0	NULL	MR imaging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	MR imaging was able to depict the extent and progression of myelination , and it may be used to continue follow-up of these patients beyond the time of fontanel closure .
	manualset3
224061	2	420910	7	NULL	NULL	0	NULL	extent 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MR imaging was able to depict the extent and progression of myelination , and it may be used to continue follow-up of these patients beyond the time of fontanel closure .
	manualset3
224062	3	420910	7	NULL	NULL	0	NULL	progression 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MR imaging was able to depict the extent and progression of myelination , and it may be used to continue follow-up of these patients beyond the time of fontanel closure .
	manualset3
224063	4	420910	7	NULL	NULL	0	NULL	 myelination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MR imaging was able to depict the extent and progression of myelination , and it may be used to continue follow-up of these patients beyond the time of fontanel closure .
	manualset3
224064	5	420910	7	NULL	NULL	0	NULL	 follow-up 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MR imaging was able to depict the extent and progression of myelination , and it may be used to continue follow-up of these patients beyond the time of fontanel closure .
	manualset3
224065	6	420910	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	MR imaging was able to depict the extent and progression of myelination , and it may be used to continue follow-up of these patients beyond the time of fontanel closure .
	manualset3
224066	7	420910	7	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	MR imaging was able to depict the extent and progression of myelination , and it may be used to continue follow-up of these patients beyond the time of fontanel closure .
	manualset3
224067	8	420910	7	NULL	NULL	0	NULL	fontanel closure 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MR imaging was able to depict the extent and progression of myelination , and it may be used to continue follow-up of these patients beyond the time of fontanel closure .
	manualset3
224068	1	420911	7	NULL	NULL	0	NULL	Postsurgical irradiation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Postsurgical irradiation is the most effective treatment currently available for improving survival .
	manualset3
224069	2	420911	7	NULL	NULL	0	NULL	effective treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Postsurgical irradiation is the most effective treatment currently available for improving survival .
	manualset3
224070	3	420911	7	NULL	NULL	0	NULL	survival 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Postsurgical irradiation is the most effective treatment currently available for improving survival .
	manualset3
224071	1	420912	7	NULL	NULL	0	NULL	Cytomegalovirus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Cytomegalovirus in the brain : in vitro infection of human brain-derived cells .
	manualset3
224072	2	420912	7	NULL	NULL	0	NULL	 brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Cytomegalovirus in the brain : in vitro infection of human brain-derived cells .
	manualset3
224073	3	420912	7	NULL	NULL	0	NULL	in vitro infection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cytomegalovirus in the brain : in vitro infection of human brain-derived cells .
	manualset3
224074	4	420912	7	NULL	NULL	0	NULL	human brain-derived cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Cytomegalovirus in the brain : in vitro infection of human brain-derived cells .
	manualset3
224075	1	420913	7	NULL	NULL	0	NULL	 increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in ( K + ) o evoked by 6 Hz stimulation was elevated in 10 mM-K + medium ( 133 % of that in 5 mM-K + medium ) and reduced in 0 mM-K + medium and in 25 mM-K + medium .
	manualset3
224076	2	420913	7	NULL	NULL	0	NULL	( K + ) o	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in ( K + ) o evoked by 6 Hz stimulation was elevated in 10 mM-K + medium ( 133 % of that in 5 mM-K + medium ) and reduced in 0 mM-K + medium and in 25 mM-K + medium .
	manualset3
224077	3	420913	7	NULL	NULL	0	NULL	6 Hz stimulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in ( K + ) o evoked by 6 Hz stimulation was elevated in 10 mM-K + medium ( 133 % of that in 5 mM-K + medium ) and reduced in 0 mM-K + medium and in 25 mM-K + medium .
	manualset3
224078	4	420913	7	NULL	NULL	0	NULL	10 mM-K + medium	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in ( K + ) o evoked by 6 Hz stimulation was elevated in 10 mM-K + medium ( 133 % of that in 5 mM-K + medium ) and reduced in 0 mM-K + medium and in 25 mM-K + medium .
	manualset3
224079	5	420913	7	NULL	NULL	0	NULL	133 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in ( K + ) o evoked by 6 Hz stimulation was elevated in 10 mM-K + medium ( 133 % of that in 5 mM-K + medium ) and reduced in 0 mM-K + medium and in 25 mM-K + medium .
	manualset3
224080	6	420913	7	NULL	NULL	0	NULL	5 mM-K + medium	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in ( K + ) o evoked by 6 Hz stimulation was elevated in 10 mM-K + medium ( 133 % of that in 5 mM-K + medium ) and reduced in 0 mM-K + medium and in 25 mM-K + medium .
	manualset3
224081	7	420913	7	NULL	NULL	0	NULL	0 mM-K + medium	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in ( K + ) o evoked by 6 Hz stimulation was elevated in 10 mM-K + medium ( 133 % of that in 5 mM-K + medium ) and reduced in 0 mM-K + medium and in 25 mM-K + medium .
	manualset3
224082	8	420913	7	NULL	NULL	0	NULL	25 mM-K + medium 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The increase in ( K + ) o evoked by 6 Hz stimulation was elevated in 10 mM-K + medium ( 133 % of that in 5 mM-K + medium ) and reduced in 0 mM-K + medium and in 25 mM-K + medium .
	manualset3
224083	1	420914	7	NULL	NULL	0	NULL	algorithms	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We developed algorithms for a straightforward implementation of an automated , time-resolved reconstruction of the membrane conformations from RICM/DW-RICM images , taking into account all the interfaces in the system and blurring of the data due to camera noise .
	manualset3
224084	2	420914	7	NULL	NULL	0	NULL	straightforward implementation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We developed algorithms for a straightforward implementation of an automated , time-resolved reconstruction of the membrane conformations from RICM/DW-RICM images , taking into account all the interfaces in the system and blurring of the data due to camera noise .
	manualset3
224085	3	420914	7	NULL	NULL	0	NULL	automated , time-resolved reconstruction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We developed algorithms for a straightforward implementation of an automated , time-resolved reconstruction of the membrane conformations from RICM/DW-RICM images , taking into account all the interfaces in the system and blurring of the data due to camera noise .
	manualset3
224086	4	420914	7	NULL	NULL	0	NULL	membrane conformations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We developed algorithms for a straightforward implementation of an automated , time-resolved reconstruction of the membrane conformations from RICM/DW-RICM images , taking into account all the interfaces in the system and blurring of the data due to camera noise .
	manualset3
224087	5	420914	7	NULL	NULL	0	NULL	RICM/DW-RICM images	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We developed algorithms for a straightforward implementation of an automated , time-resolved reconstruction of the membrane conformations from RICM/DW-RICM images , taking into account all the interfaces in the system and blurring of the data due to camera noise .
	manualset3
224088	6	420914	7	NULL	NULL	0	NULL	account	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We developed algorithms for a straightforward implementation of an automated , time-resolved reconstruction of the membrane conformations from RICM/DW-RICM images , taking into account all the interfaces in the system and blurring of the data due to camera noise .
	manualset3
224089	7	420914	7	NULL	NULL	0	NULL	interfaces 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We developed algorithms for a straightforward implementation of an automated , time-resolved reconstruction of the membrane conformations from RICM/DW-RICM images , taking into account all the interfaces in the system and blurring of the data due to camera noise .
	manualset3
224090	8	420914	7	NULL	NULL	0	NULL	system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	We developed algorithms for a straightforward implementation of an automated , time-resolved reconstruction of the membrane conformations from RICM/DW-RICM images , taking into account all the interfaces in the system and blurring of the data due to camera noise .
	manualset3
224091	9	420914	7	NULL	NULL	0	NULL	blurring	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We developed algorithms for a straightforward implementation of an automated , time-resolved reconstruction of the membrane conformations from RICM/DW-RICM images , taking into account all the interfaces in the system and blurring of the data due to camera noise .
	manualset3
224092	10	420914	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	We developed algorithms for a straightforward implementation of an automated , time-resolved reconstruction of the membrane conformations from RICM/DW-RICM images , taking into account all the interfaces in the system and blurring of the data due to camera noise .
	manualset3
224093	11	420914	7	NULL	NULL	0	NULL	camera noise 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We developed algorithms for a straightforward implementation of an automated , time-resolved reconstruction of the membrane conformations from RICM/DW-RICM images , taking into account all the interfaces in the system and blurring of the data due to camera noise .
	manualset3
224094	1	420915	7	NULL	NULL	0	NULL	CAR activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	CAR activation results in the transcriptional induction of numerous hepatic genes including those that encode xenobiotic-metabolizing enzymes such as a set of cytochrome P450s .
	manualset3
224095	2	420915	7	NULL	NULL	0	NULL	transcriptional induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	CAR activation results in the transcriptional induction of numerous hepatic genes including those that encode xenobiotic-metabolizing enzymes such as a set of cytochrome P450s .
	manualset3
224096	3	420915	7	NULL	NULL	0	NULL	hepatic genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	CAR activation results in the transcriptional induction of numerous hepatic genes including those that encode xenobiotic-metabolizing enzymes such as a set of cytochrome P450s .
	manualset3
224097	4	420915	7	NULL	NULL	0	NULL	xenobiotic-metabolizing enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	CAR activation results in the transcriptional induction of numerous hepatic genes including those that encode xenobiotic-metabolizing enzymes such as a set of cytochrome P450s .
	manualset3
224098	5	420915	7	NULL	NULL	0	NULL	set	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	CAR activation results in the transcriptional induction of numerous hepatic genes including those that encode xenobiotic-metabolizing enzymes such as a set of cytochrome P450s .
	manualset3
224099	6	420915	7	NULL	NULL	0	NULL	cytochrome P450s	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	CAR activation results in the transcriptional induction of numerous hepatic genes including those that encode xenobiotic-metabolizing enzymes such as a set of cytochrome P450s .
	manualset3
224100	1	420916	7	NULL	NULL	0	NULL	account	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On one account , congruency is explained by the match between position and a mental simulation of meaning .
	manualset3
224101	2	420916	7	NULL	NULL	0	NULL	congruency	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On one account , congruency is explained by the match between position and a mental simulation of meaning .
	manualset3
224102	3	420916	7	NULL	NULL	0	NULL	match 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On one account , congruency is explained by the match between position and a mental simulation of meaning .
	manualset3
224103	4	420916	7	NULL	NULL	0	NULL	position	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	On one account , congruency is explained by the match between position and a mental simulation of meaning .
	manualset3
224104	5	420916	7	NULL	NULL	0	NULL	mental simulation	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On one account , congruency is explained by the match between position and a mental simulation of meaning .
	manualset3
224105	6	420916	7	NULL	NULL	0	NULL	meaning 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On one account , congruency is explained by the match between position and a mental simulation of meaning .
	manualset3
225417	7	420916	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On one account , congruency is explained by the match between position and a mental simulation of meaning .
	manualset3
224106	1	420917	7	NULL	NULL	0	NULL	phenomenon	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The phenomenon of lowering a seizure readiness level after frequent audiogenic seizures in Krushinski-Molodkina rats ) .
	manualset3
224107	2	420917	7	NULL	NULL	0	NULL	seizure readiness level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( The phenomenon of lowering a seizure readiness level after frequent audiogenic seizures in Krushinski-Molodkina rats ) .
	manualset3
224108	3	420917	7	NULL	NULL	0	NULL	 frequent audiogenic seizures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( The phenomenon of lowering a seizure readiness level after frequent audiogenic seizures in Krushinski-Molodkina rats ) .
	manualset3
224109	4	420917	7	NULL	NULL	0	NULL	Krushinski-Molodkina rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( The phenomenon of lowering a seizure readiness level after frequent audiogenic seizures in Krushinski-Molodkina rats ) .
	manualset3
224110	1	420918	7	NULL	NULL	0	NULL	 hand-specific component	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A smaller but significant , nontransferable , and hand-specific component was evident in each session and did not increase with practice .
	manualset3
224113	2	420918	7	NULL	NULL	0	NULL	session	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A smaller but significant , nontransferable , and hand-specific component was evident in each session and did not increase with practice .
	manualset3
224114	3	420918	7	NULL	NULL	0	NULL	practice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A smaller but significant , nontransferable , and hand-specific component was evident in each session and did not increase with practice .
	manualset3
224115	1	420919	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , biophysical variability alone reduced pair-wise output spike correlations to low levels .
	manualset3
224116	2	420919	7	NULL	NULL	0	NULL	biophysical variability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , biophysical variability alone reduced pair-wise output spike correlations to low levels .
	manualset3
224117	3	420919	7	NULL	NULL	0	NULL	pair-wise output spike correlations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , biophysical variability alone reduced pair-wise output spike correlations to low levels .
	manualset3
224118	4	420919	7	NULL	NULL	0	NULL	low levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , biophysical variability alone reduced pair-wise output spike correlations to low levels .
	manualset3
224119	1	420920	7	NULL	NULL	0	NULL	blacks 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	This applied to both blacks and whites when examined for the early years of the reproductive cycle .
	manualset3
224120	2	420920	7	NULL	NULL	0	NULL	whites	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	This applied to both blacks and whites when examined for the early years of the reproductive cycle .
	manualset3
224121	3	420920	7	NULL	NULL	0	NULL	early years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	This applied to both blacks and whites when examined for the early years of the reproductive cycle .
	manualset3
224122	4	420920	7	NULL	NULL	0	NULL	 reproductive cycle	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This applied to both blacks and whites when examined for the early years of the reproductive cycle .
	manualset3
224123	1	420921	7	NULL	NULL	0	NULL	nutrition 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The nutrition of the gastrectomite .
	manualset3
224124	2	420921	7	NULL	NULL	0	NULL	gastrectomite 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The nutrition of the gastrectomite .
	manualset3
224125	1	420922	7	NULL	NULL	0	NULL	interest	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore found it of interest to test a new system for capillary blood collection , storage and transportation , which makes it possible to perform capillary blood collection at home , and then forward the blood sample for the laboratory assay of glycated hemoglobin .
	manualset3
224126	2	420922	7	NULL	NULL	0	NULL	 test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore found it of interest to test a new system for capillary blood collection , storage and transportation , which makes it possible to perform capillary blood collection at home , and then forward the blood sample for the laboratory assay of glycated hemoglobin .
	manualset3
224127	3	420922	7	NULL	NULL	0	NULL	new system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore found it of interest to test a new system for capillary blood collection , storage and transportation , which makes it possible to perform capillary blood collection at home , and then forward the blood sample for the laboratory assay of glycated hemoglobin .
	manualset3
224128	4	420922	7	NULL	NULL	0	NULL	capillary blood collection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore found it of interest to test a new system for capillary blood collection , storage and transportation , which makes it possible to perform capillary blood collection at home , and then forward the blood sample for the laboratory assay of glycated hemoglobin .
	manualset3
224129	5	420922	7	NULL	NULL	0	NULL	storage 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore found it of interest to test a new system for capillary blood collection , storage and transportation , which makes it possible to perform capillary blood collection at home , and then forward the blood sample for the laboratory assay of glycated hemoglobin .
	manualset3
224130	6	420922	7	NULL	NULL	0	NULL	 transportation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore found it of interest to test a new system for capillary blood collection , storage and transportation , which makes it possible to perform capillary blood collection at home , and then forward the blood sample for the laboratory assay of glycated hemoglobin .
	manualset3
224131	7	420922	7	NULL	NULL	0	NULL	capillary blood collection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore found it of interest to test a new system for capillary blood collection , storage and transportation , which makes it possible to perform capillary blood collection at home , and then forward the blood sample for the laboratory assay of glycated hemoglobin .
	manualset3
224132	8	420922	7	NULL	NULL	0	NULL	home	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore found it of interest to test a new system for capillary blood collection , storage and transportation , which makes it possible to perform capillary blood collection at home , and then forward the blood sample for the laboratory assay of glycated hemoglobin .
	manualset3
224133	9	420922	7	NULL	NULL	0	NULL	blood sample	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore found it of interest to test a new system for capillary blood collection , storage and transportation , which makes it possible to perform capillary blood collection at home , and then forward the blood sample for the laboratory assay of glycated hemoglobin .
	manualset3
224134	10	420922	7	NULL	NULL	0	NULL	laboratory assay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore found it of interest to test a new system for capillary blood collection , storage and transportation , which makes it possible to perform capillary blood collection at home , and then forward the blood sample for the laboratory assay of glycated hemoglobin .
	manualset3
224135	11	420922	7	NULL	NULL	0	NULL	glycated hemoglobin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We therefore found it of interest to test a new system for capillary blood collection , storage and transportation , which makes it possible to perform capillary blood collection at home , and then forward the blood sample for the laboratory assay of glycated hemoglobin .
	manualset3
224136	1	420923	7	NULL	NULL	0	NULL	 EEG	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , both EEG and behavioural changes during drowsiness often exhibit stereotyped 18-s cycles .
	manualset3
224137	2	420923	7	NULL	NULL	0	NULL	behavioural changes	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , both EEG and behavioural changes during drowsiness often exhibit stereotyped 18-s cycles .
	manualset3
224138	3	420923	7	NULL	NULL	0	NULL	drowsiness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , both EEG and behavioural changes during drowsiness often exhibit stereotyped 18-s cycles .
	manualset3
224139	4	420923	7	NULL	NULL	0	NULL	stereotyped 18-s cycles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , both EEG and behavioural changes during drowsiness often exhibit stereotyped 18-s cycles .
	manualset3
224140	1	420924	7	NULL	NULL	0	NULL	Choleretic potency 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Choleretic potency of bile acids ; statistical analysis ) .
	manualset3
224141	2	420924	7	NULL	NULL	0	NULL	bile acids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Choleretic potency of bile acids ; statistical analysis ) .
	manualset3
224142	3	420924	7	NULL	NULL	0	NULL	statistical analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Choleretic potency of bile acids ; statistical analysis ) .
	manualset3
224143	1	420925	7	NULL	NULL	0	NULL	cGMP-specific PDEs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the cGMP-specific PDEs , PDE5 is quantitatively prevalent in lung tissue .
	manualset3
224144	2	420925	7	NULL	NULL	0	NULL	PDE5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the cGMP-specific PDEs , PDE5 is quantitatively prevalent in lung tissue .
	manualset3
224145	3	420925	7	NULL	NULL	0	NULL	lung tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the cGMP-specific PDEs , PDE5 is quantitatively prevalent in lung tissue .
	manualset3
224146	1	420926	7	NULL	NULL	0	NULL	Permeability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Permeability of the abdominal nerve cord of the American cockroach , Periplaneta americana ( L. ) to aliphatic alcohols .
	manualset3
224147	2	420926	7	NULL	NULL	0	NULL	abdominal nerve cord 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Permeability of the abdominal nerve cord of the American cockroach , Periplaneta americana ( L. ) to aliphatic alcohols .
	manualset3
224148	3	420926	7	NULL	NULL	0	NULL	American cockroach 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Permeability of the abdominal nerve cord of the American cockroach , Periplaneta americana ( L. ) to aliphatic alcohols .
	manualset3
224149	4	420926	7	NULL	NULL	0	NULL	Periplaneta americana ( L. )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Permeability of the abdominal nerve cord of the American cockroach , Periplaneta americana ( L. ) to aliphatic alcohols .
	manualset3
224150	5	420926	7	NULL	NULL	0	NULL	aliphatic alcohols	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Permeability of the abdominal nerve cord of the American cockroach , Periplaneta americana ( L. ) to aliphatic alcohols .
	manualset3
224151	1	420927	7	NULL	NULL	0	NULL	degree	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of rotational mobility in accordance with the carbon atom numbers of phospholipids comprising neuronal and model membranes was in the order at the 16 , 12 , 9 , 6 and 2 position of aliphatic chain present in phospholipids .
	manualset3
224152	2	420927	7	NULL	NULL	0	NULL	 rotational mobility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of rotational mobility in accordance with the carbon atom numbers of phospholipids comprising neuronal and model membranes was in the order at the 16 , 12 , 9 , 6 and 2 position of aliphatic chain present in phospholipids .
	manualset3
224153	3	420927	7	NULL	NULL	0	NULL	carbon atom numbers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of rotational mobility in accordance with the carbon atom numbers of phospholipids comprising neuronal and model membranes was in the order at the 16 , 12 , 9 , 6 and 2 position of aliphatic chain present in phospholipids .
	manualset3
224154	4	420927	7	NULL	NULL	0	NULL	phospholipids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of rotational mobility in accordance with the carbon atom numbers of phospholipids comprising neuronal and model membranes was in the order at the 16 , 12 , 9 , 6 and 2 position of aliphatic chain present in phospholipids .
	manualset3
224155	5	420927	7	NULL	NULL	0	NULL	neuronal membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of rotational mobility in accordance with the carbon atom numbers of phospholipids comprising neuronal and model membranes was in the order at the 16 , 12 , 9 , 6 and 2 position of aliphatic chain present in phospholipids .
	manualset3
224156	6	420927	7	NULL	NULL	0	NULL	model membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of rotational mobility in accordance with the carbon atom numbers of phospholipids comprising neuronal and model membranes was in the order at the 16 , 12 , 9 , 6 and 2 position of aliphatic chain present in phospholipids .
	manualset3
224157	7	420927	7	NULL	NULL	0	NULL	 order	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of rotational mobility in accordance with the carbon atom numbers of phospholipids comprising neuronal and model membranes was in the order at the 16 , 12 , 9 , 6 and 2 position of aliphatic chain present in phospholipids .
	manualset3
224158	8	420927	7	NULL	NULL	0	NULL	16 position	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of rotational mobility in accordance with the carbon atom numbers of phospholipids comprising neuronal and model membranes was in the order at the 16 , 12 , 9 , 6 and 2 position of aliphatic chain present in phospholipids .
	manualset3
224159	9	420927	7	NULL	NULL	0	NULL	12 position	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of rotational mobility in accordance with the carbon atom numbers of phospholipids comprising neuronal and model membranes was in the order at the 16 , 12 , 9 , 6 and 2 position of aliphatic chain present in phospholipids .
	manualset3
224160	10	420927	7	NULL	NULL	0	NULL	9 position	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of rotational mobility in accordance with the carbon atom numbers of phospholipids comprising neuronal and model membranes was in the order at the 16 , 12 , 9 , 6 and 2 position of aliphatic chain present in phospholipids .
	manualset3
224161	11	420927	7	NULL	NULL	0	NULL	6 position	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of rotational mobility in accordance with the carbon atom numbers of phospholipids comprising neuronal and model membranes was in the order at the 16 , 12 , 9 , 6 and 2 position of aliphatic chain present in phospholipids .
	manualset3
224162	12	420927	7	NULL	NULL	0	NULL	2 position 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of rotational mobility in accordance with the carbon atom numbers of phospholipids comprising neuronal and model membranes was in the order at the 16 , 12 , 9 , 6 and 2 position of aliphatic chain present in phospholipids .
	manualset3
224163	13	420927	7	NULL	NULL	0	NULL	aliphatic chain 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of rotational mobility in accordance with the carbon atom numbers of phospholipids comprising neuronal and model membranes was in the order at the 16 , 12 , 9 , 6 and 2 position of aliphatic chain present in phospholipids .
	manualset3
224164	14	420927	7	NULL	NULL	0	NULL	phospholipids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The degree of rotational mobility in accordance with the carbon atom numbers of phospholipids comprising neuronal and model membranes was in the order at the 16 , 12 , 9 , 6 and 2 position of aliphatic chain present in phospholipids .
	manualset3
224165	1	420928	7	NULL	NULL	0	NULL	Speleotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Speleotherapy was conducted in 24-day courses in salt caves of Chon-Tuz ( 2100 m above the sea level ) .
	manualset3
224166	2	420928	7	NULL	NULL	0	NULL	24-day courses	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Speleotherapy was conducted in 24-day courses in salt caves of Chon-Tuz ( 2100 m above the sea level ) .
	manualset3
224167	3	420928	7	NULL	NULL	0	NULL	salt caves	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Speleotherapy was conducted in 24-day courses in salt caves of Chon-Tuz ( 2100 m above the sea level ) .
	manualset3
224168	4	420928	7	NULL	NULL	0	NULL	Chon-Tuz	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Speleotherapy was conducted in 24-day courses in salt caves of Chon-Tuz ( 2100 m above the sea level ) .
	manualset3
224169	5	420928	7	NULL	NULL	0	NULL	2100 m	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Speleotherapy was conducted in 24-day courses in salt caves of Chon-Tuz ( 2100 m above the sea level ) .
	manualset3
224170	6	420928	7	NULL	NULL	0	NULL	sea level	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Speleotherapy was conducted in 24-day courses in salt caves of Chon-Tuz ( 2100 m above the sea level ) .
	manualset3
224171	1	420929	7	NULL	NULL	0	NULL	course 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After a course of TACE , the tumor became markedly enlarged and was accompanied by a PVTT ( Vp4 ) .
	manualset3
224172	2	420929	7	NULL	NULL	0	NULL	TACE	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After a course of TACE , the tumor became markedly enlarged and was accompanied by a PVTT ( Vp4 ) .
	manualset3
224173	3	420929	7	NULL	NULL	0	NULL	tumor	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	After a course of TACE , the tumor became markedly enlarged and was accompanied by a PVTT ( Vp4 ) .
	manualset3
224174	4	420929	7	NULL	NULL	0	NULL	PVTT ( Vp4 )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	After a course of TACE , the tumor became markedly enlarged and was accompanied by a PVTT ( Vp4 ) .
	manualset3
224175	1	420930	7	NULL	NULL	0	NULL	inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All produced inhibition except for the ampholytic detergent , miranol H2M which was not inhibitory .
	manualset3
224176	2	420930	7	NULL	NULL	0	NULL	ampholytic detergent 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All produced inhibition except for the ampholytic detergent , miranol H2M which was not inhibitory .
	manualset3
224177	3	420930	7	NULL	NULL	0	NULL	miranol H2M	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All produced inhibition except for the ampholytic detergent , miranol H2M which was not inhibitory .
	manualset3
224272	1	420931	7	NULL	NULL	0	NULL	randomized , blind , placebo-controlled , 4-arm clinical trial	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We performed a randomized , blind , placebo-controlled , 4-arm clinical trial to determine the effects of DCS and VPA on the overnight properties of declarative and procedural learning in 60 healthy adults .
	manualset3
224275	2	420931	7	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We performed a randomized , blind , placebo-controlled , 4-arm clinical trial to determine the effects of DCS and VPA on the overnight properties of declarative and procedural learning in 60 healthy adults .
	manualset3
224277	3	420931	7	NULL	NULL	0	NULL	DCS	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We performed a randomized , blind , placebo-controlled , 4-arm clinical trial to determine the effects of DCS and VPA on the overnight properties of declarative and procedural learning in 60 healthy adults .
	manualset3
224278	4	420931	7	NULL	NULL	0	NULL	VPA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We performed a randomized , blind , placebo-controlled , 4-arm clinical trial to determine the effects of DCS and VPA on the overnight properties of declarative and procedural learning in 60 healthy adults .
	manualset3
224279	5	420931	7	NULL	NULL	0	NULL	overnight properties	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We performed a randomized , blind , placebo-controlled , 4-arm clinical trial to determine the effects of DCS and VPA on the overnight properties of declarative and procedural learning in 60 healthy adults .
	manualset3
224280	6	420931	7	NULL	NULL	0	NULL	declarative learning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We performed a randomized , blind , placebo-controlled , 4-arm clinical trial to determine the effects of DCS and VPA on the overnight properties of declarative and procedural learning in 60 healthy adults .
	manualset3
224281	7	420931	7	NULL	NULL	0	NULL	procedural learning 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We performed a randomized , blind , placebo-controlled , 4-arm clinical trial to determine the effects of DCS and VPA on the overnight properties of declarative and procedural learning in 60 healthy adults .
	manualset3
224282	8	420931	7	NULL	NULL	0	NULL	60 healthy adults .	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We performed a randomized , blind , placebo-controlled , 4-arm clinical trial to determine the effects of DCS and VPA on the overnight properties of declarative and procedural learning in 60 healthy adults .
	manualset3
224285	1	420932	7	NULL	NULL	0	NULL	 advantages 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we review the advantages afforded by lentivirus-mediated globin gene transfer and recent studies based on this strategy .
	manualset3
224286	2	420932	7	NULL	NULL	0	NULL	lentivirus-mediated globin gene transfer	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we review the advantages afforded by lentivirus-mediated globin gene transfer and recent studies based on this strategy .
	manualset3
224287	3	420932	7	NULL	NULL	0	NULL	recent studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we review the advantages afforded by lentivirus-mediated globin gene transfer and recent studies based on this strategy .
	manualset3
224288	4	420932	7	NULL	NULL	0	NULL	strategy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we review the advantages afforded by lentivirus-mediated globin gene transfer and recent studies based on this strategy .
	manualset3
224289	1	420933	7	NULL	NULL	0	NULL	amine groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To introduce amine groups , ELP was modified with lysine for conjugation with PS microbeads functionalized with carboxylic groups .
	manualset3
224290	2	420933	7	NULL	NULL	0	NULL	ELP	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	To introduce amine groups , ELP was modified with lysine for conjugation with PS microbeads functionalized with carboxylic groups .
	manualset3
224291	3	420933	7	NULL	NULL	0	NULL	 lysine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To introduce amine groups , ELP was modified with lysine for conjugation with PS microbeads functionalized with carboxylic groups .
	manualset3
224292	4	420933	7	NULL	NULL	0	NULL	conjugation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To introduce amine groups , ELP was modified with lysine for conjugation with PS microbeads functionalized with carboxylic groups .
	manualset3
224293	5	420933	7	NULL	NULL	0	NULL	PS microbeads	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To introduce amine groups , ELP was modified with lysine for conjugation with PS microbeads functionalized with carboxylic groups .
	manualset3
224294	6	420933	7	NULL	NULL	0	NULL	carboxylic groups 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	To introduce amine groups , ELP was modified with lysine for conjugation with PS microbeads functionalized with carboxylic groups .
	manualset3
224295	1	420934	7	NULL	NULL	0	NULL	coagulase-negative staphylococci	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the coagulase-negative staphylococci , false-positive results were seen with strains of S. capitis .
	manualset3
224296	2	420934	7	NULL	NULL	0	NULL	false-positive results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the coagulase-negative staphylococci , false-positive results were seen with strains of S. capitis .
	manualset3
224297	3	420934	7	NULL	NULL	0	NULL	strains 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the coagulase-negative staphylococci , false-positive results were seen with strains of S. capitis .
	manualset3
224298	4	420934	7	NULL	NULL	0	NULL	S. capitis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the coagulase-negative staphylococci , false-positive results were seen with strains of S. capitis .
	manualset3
224299	1	420935	7	NULL	NULL	0	NULL	Ancillary autoantibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ancillary autoantibodies that enhance diagnostic specificity , have prognostic connotation , or direct treatment are antibodies to endomysium , tissue transglutaminase , histones , doubled-stranded DNA , and actin .
	manualset3
224300	2	420935	7	NULL	NULL	0	NULL	diagnostic specificity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ancillary autoantibodies that enhance diagnostic specificity , have prognostic connotation , or direct treatment are antibodies to endomysium , tissue transglutaminase , histones , doubled-stranded DNA , and actin .
	manualset3
224301	3	420935	7	NULL	NULL	0	NULL	prognostic connotation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ancillary autoantibodies that enhance diagnostic specificity , have prognostic connotation , or direct treatment are antibodies to endomysium , tissue transglutaminase , histones , doubled-stranded DNA , and actin .
	manualset3
224302	4	420935	7	NULL	NULL	0	NULL	direct treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ancillary autoantibodies that enhance diagnostic specificity , have prognostic connotation , or direct treatment are antibodies to endomysium , tissue transglutaminase , histones , doubled-stranded DNA , and actin .
	manualset3
224303	5	420935	7	NULL	NULL	0	NULL	antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ancillary autoantibodies that enhance diagnostic specificity , have prognostic connotation , or direct treatment are antibodies to endomysium , tissue transglutaminase , histones , doubled-stranded DNA , and actin .
	manualset3
224304	6	420935	7	NULL	NULL	0	NULL	endomysium 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ancillary autoantibodies that enhance diagnostic specificity , have prognostic connotation , or direct treatment are antibodies to endomysium , tissue transglutaminase , histones , doubled-stranded DNA , and actin .
	manualset3
224305	7	420935	7	NULL	NULL	0	NULL	tissue transglutaminase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Ancillary autoantibodies that enhance diagnostic specificity , have prognostic connotation , or direct treatment are antibodies to endomysium , tissue transglutaminase , histones , doubled-stranded DNA , and actin .
	manualset3
224306	8	420935	7	NULL	NULL	0	NULL	histones	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ancillary autoantibodies that enhance diagnostic specificity , have prognostic connotation , or direct treatment are antibodies to endomysium , tissue transglutaminase , histones , doubled-stranded DNA , and actin .
	manualset3
224307	9	420935	7	NULL	NULL	0	NULL	doubled-stranded DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Ancillary autoantibodies that enhance diagnostic specificity , have prognostic connotation , or direct treatment are antibodies to endomysium , tissue transglutaminase , histones , doubled-stranded DNA , and actin .
	manualset3
224308	10	420935	7	NULL	NULL	0	NULL	actin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Ancillary autoantibodies that enhance diagnostic specificity , have prognostic connotation , or direct treatment are antibodies to endomysium , tissue transglutaminase , histones , doubled-stranded DNA , and actin .
	manualset3
224309	1	420936	7	NULL	NULL	0	NULL	memory	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We then examined whether memory of a sequential procedure depends on the entire sequence , not individual stimulus sets .
	manualset3
224310	2	420936	7	NULL	NULL	0	NULL	sequential procedure	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We then examined whether memory of a sequential procedure depends on the entire sequence , not individual stimulus sets .
	manualset3
224311	3	420936	7	NULL	NULL	0	NULL	entire sequence	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	We then examined whether memory of a sequential procedure depends on the entire sequence , not individual stimulus sets .
	manualset3
224312	4	420936	7	NULL	NULL	0	NULL	individual stimulus sets	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We then examined whether memory of a sequential procedure depends on the entire sequence , not individual stimulus sets .
	manualset3
224313	1	420937	7	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of kojic acid produced by the intact mycelia was found to be more than that produced by the disrupted mycelia .
	manualset3
224314	2	420937	7	NULL	NULL	0	NULL	kojic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of kojic acid produced by the intact mycelia was found to be more than that produced by the disrupted mycelia .
	manualset3
224315	3	420937	7	NULL	NULL	0	NULL	 intact mycelia 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of kojic acid produced by the intact mycelia was found to be more than that produced by the disrupted mycelia .
	manualset3
224316	4	420937	7	NULL	NULL	0	NULL	disrupted mycelia	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of kojic acid produced by the intact mycelia was found to be more than that produced by the disrupted mycelia .
	manualset3
224317	1	420938	7	NULL	NULL	0	NULL	INTENSITY 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	THE INTENSITY AND SPECTRAL DISTRIBUTION OF SCATTERED RADIATION FROM COBALT-60 SOURCES .
	manualset3
224318	2	420938	7	NULL	NULL	0	NULL	SPECTRAL DISTRIBUTION	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	THE INTENSITY AND SPECTRAL DISTRIBUTION OF SCATTERED RADIATION FROM COBALT-60 SOURCES .
	manualset3
224319	3	420938	7	NULL	NULL	NULL	NULL	SCATTERED RADIATION	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	THE INTENSITY AND SPECTRAL DISTRIBUTION OF SCATTERED RADIATION FROM COBALT-60 SOURCES .
	manualset3
224320	4	420938	7	NULL	NULL	0	NULL	COBALT-60 SOURCES 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	THE INTENSITY AND SPECTRAL DISTRIBUTION OF SCATTERED RADIATION FROM COBALT-60 SOURCES .
	manualset3
224321	1	420939	7	NULL	NULL	0	NULL	Electrophysiological study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Electrophysiological study of the topographical organization of the lateral Deiter 's vestibular nucleus ) .
	manualset3
224322	2	420939	7	NULL	NULL	0	NULL	 topographical organization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Electrophysiological study of the topographical organization of the lateral Deiter 's vestibular nucleus ) .
	manualset3
224323	3	420939	7	NULL	NULL	NULL	NULL	lateral Deiter 's vestibular nucleus	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Electrophysiological study of the topographical organization of the lateral Deiter 's vestibular nucleus ) .
	manualset3
224324	1	420940	7	NULL	NULL	0	NULL	homocysteine levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , we found that homocysteine levels were 11.2 + / - 5 micromol/l for no consumption , 11.7 + / - 7 micromol/l for & lt ; 100 ml/day , 12.5 + / - 7 micromol/l for 200-400 ml/day , and 12.7 + / - 4 micromol/l for ) 500 ml/day consumption ( P = 0.018 ) .
	manualset3
224325	2	420940	7	NULL	NULL	0	NULL	11.2 + / - 5 micromol/l	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , we found that homocysteine levels were 11.2 + / - 5 micromol/l for no consumption , 11.7 + / - 7 micromol/l for & lt ; 100 ml/day , 12.5 + / - 7 micromol/l for 200-400 ml/day , and 12.7 + / - 4 micromol/l for ) 500 ml/day consumption ( P = 0.018 ) .
	manualset3
224326	3	420940	7	NULL	NULL	0	NULL	no consumption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , we found that homocysteine levels were 11.2 + / - 5 micromol/l for no consumption , 11.7 + / - 7 micromol/l for & lt ; 100 ml/day , 12.5 + / - 7 micromol/l for 200-400 ml/day , and 12.7 + / - 4 micromol/l for ) 500 ml/day consumption ( P = 0.018 ) .
	manualset3
224327	4	420940	7	NULL	NULL	0	NULL	 11.7 + / - 7 micromol/	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , we found that homocysteine levels were 11.2 + / - 5 micromol/l for no consumption , 11.7 + / - 7 micromol/l for & lt ; 100 ml/day , 12.5 + / - 7 micromol/l for 200-400 ml/day , and 12.7 + / - 4 micromol/l for ) 500 ml/day consumption ( P = 0.018 ) .
	manualset3
224328	5	420940	7	NULL	NULL	NULL	NULL	& lt ; 100 ml/day	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In particular , we found that homocysteine levels were 11.2 + / - 5 micromol/l for no consumption , 11.7 + / - 7 micromol/l for & lt ; 100 ml/day , 12.5 + / - 7 micromol/l for 200-400 ml/day , and 12.7 + / - 4 micromol/l for ) 500 ml/day consumption ( P = 0.018 ) .
	manualset3
224329	6	420940	7	NULL	NULL	0	NULL	12.5 + / - 7 micromol/l	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , we found that homocysteine levels were 11.2 + / - 5 micromol/l for no consumption , 11.7 + / - 7 micromol/l for & lt ; 100 ml/day , 12.5 + / - 7 micromol/l for 200-400 ml/day , and 12.7 + / - 4 micromol/l for ) 500 ml/day consumption ( P = 0.018 ) .
	manualset3
224330	7	420940	7	NULL	NULL	0	NULL	200-400 ml/day	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , we found that homocysteine levels were 11.2 + / - 5 micromol/l for no consumption , 11.7 + / - 7 micromol/l for & lt ; 100 ml/day , 12.5 + / - 7 micromol/l for 200-400 ml/day , and 12.7 + / - 4 micromol/l for ) 500 ml/day consumption ( P = 0.018 ) .
	manualset3
224331	8	420940	7	NULL	NULL	0	NULL	12.7 + / - 4 micromol/l	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , we found that homocysteine levels were 11.2 + / - 5 micromol/l for no consumption , 11.7 + / - 7 micromol/l for & lt ; 100 ml/day , 12.5 + / - 7 micromol/l for 200-400 ml/day , and 12.7 + / - 4 micromol/l for ) 500 ml/day consumption ( P = 0.018 ) .
	manualset3
224333	9	420940	7	NULL	NULL	0	NULL	500 ml/day consumption	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , we found that homocysteine levels were 11.2 + / - 5 micromol/l for no consumption , 11.7 + / - 7 micromol/l for & lt ; 100 ml/day , 12.5 + / - 7 micromol/l for 200-400 ml/day , and 12.7 + / - 4 micromol/l for ) 500 ml/day consumption ( P = 0.018 ) .
	manualset3
224334	10	420940	7	NULL	NULL	0	NULL	P = 0.018	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In particular , we found that homocysteine levels were 11.2 + / - 5 micromol/l for no consumption , 11.7 + / - 7 micromol/l for & lt ; 100 ml/day , 12.5 + / - 7 micromol/l for 200-400 ml/day , and 12.7 + / - 4 micromol/l for ) 500 ml/day consumption ( P = 0.018 ) .
	manualset3
224368	1	420941	7	NULL	NULL	0	NULL	evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An evaluation exclusively concerned with the way the dog families were kept showed a higher percentage of 76.2 % for litters from kennels than among those kept indoors , which amounted only to 51.4 % .
	manualset3
224369	2	420941	7	NULL	NULL	0	NULL	way	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An evaluation exclusively concerned with the way the dog families were kept showed a higher percentage of 76.2 % for litters from kennels than among those kept indoors , which amounted only to 51.4 % .
	manualset3
224370	3	420941	7	NULL	NULL	0	NULL	dog families	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	An evaluation exclusively concerned with the way the dog families were kept showed a higher percentage of 76.2 % for litters from kennels than among those kept indoors , which amounted only to 51.4 % .
	manualset3
224371	4	420941	7	NULL	NULL	0	NULL	higher percentage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An evaluation exclusively concerned with the way the dog families were kept showed a higher percentage of 76.2 % for litters from kennels than among those kept indoors , which amounted only to 51.4 % .
	manualset3
224372	5	420941	7	NULL	NULL	0	NULL	76.2 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An evaluation exclusively concerned with the way the dog families were kept showed a higher percentage of 76.2 % for litters from kennels than among those kept indoors , which amounted only to 51.4 % .
	manualset3
224373	6	420941	7	NULL	NULL	0	NULL	litters 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	An evaluation exclusively concerned with the way the dog families were kept showed a higher percentage of 76.2 % for litters from kennels than among those kept indoors , which amounted only to 51.4 % .
	manualset3
224374	7	420941	7	NULL	NULL	0	NULL	kennels	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	An evaluation exclusively concerned with the way the dog families were kept showed a higher percentage of 76.2 % for litters from kennels than among those kept indoors , which amounted only to 51.4 % .
	manualset3
224375	8	420941	7	NULL	NULL	0	NULL	 indoors	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	An evaluation exclusively concerned with the way the dog families were kept showed a higher percentage of 76.2 % for litters from kennels than among those kept indoors , which amounted only to 51.4 % .
	manualset3
224376	9	420941	7	NULL	NULL	0	NULL	 51.4 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An evaluation exclusively concerned with the way the dog families were kept showed a higher percentage of 76.2 % for litters from kennels than among those kept indoors , which amounted only to 51.4 % .
	manualset3
224377	1	420942	7	NULL	NULL	NULL	NULL	dogmas 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Among the dogmas challenged are that infection outside the home is commonplace , so-called relapse cases may in fact be largely reinfection , and active transmission may be more common than previously thought and reactivation disease relatively uncommon .
	manualset3
224378	2	420942	7	NULL	NULL	0	NULL	infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the dogmas challenged are that infection outside the home is commonplace , so-called relapse cases may in fact be largely reinfection , and active transmission may be more common than previously thought and reactivation disease relatively uncommon .
	manualset3
224379	3	420942	7	NULL	NULL	0	NULL	home	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the dogmas challenged are that infection outside the home is commonplace , so-called relapse cases may in fact be largely reinfection , and active transmission may be more common than previously thought and reactivation disease relatively uncommon .
	manualset3
224380	4	420942	7	NULL	NULL	0	NULL	commonplace	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the dogmas challenged are that infection outside the home is commonplace , so-called relapse cases may in fact be largely reinfection , and active transmission may be more common than previously thought and reactivation disease relatively uncommon .
	manualset3
224381	5	420942	7	NULL	NULL	0	NULL	relapse cases 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the dogmas challenged are that infection outside the home is commonplace , so-called relapse cases may in fact be largely reinfection , and active transmission may be more common than previously thought and reactivation disease relatively uncommon .
	manualset3
224382	6	420942	7	NULL	NULL	0	NULL	reinfection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the dogmas challenged are that infection outside the home is commonplace , so-called relapse cases may in fact be largely reinfection , and active transmission may be more common than previously thought and reactivation disease relatively uncommon .
	manualset3
224383	7	420942	7	NULL	NULL	0	NULL	active transmission 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the dogmas challenged are that infection outside the home is commonplace , so-called relapse cases may in fact be largely reinfection , and active transmission may be more common than previously thought and reactivation disease relatively uncommon .
	manualset3
224384	8	420942	7	NULL	NULL	0	NULL	reactivation disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the dogmas challenged are that infection outside the home is commonplace , so-called relapse cases may in fact be largely reinfection , and active transmission may be more common than previously thought and reactivation disease relatively uncommon .
	manualset3
224385	1	420943	7	NULL	NULL	0	NULL	Negative product value 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Negative product value for coronary artery disease is 98 % to 99 % .
	manualset3
224386	2	420943	7	NULL	NULL	0	NULL	coronary artery disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Negative product value for coronary artery disease is 98 % to 99 % .
	manualset3
224387	3	420943	7	NULL	NULL	0	NULL	98 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Negative product value for coronary artery disease is 98 % to 99 % .
	manualset3
224388	4	420943	7	NULL	NULL	0	NULL	99 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Negative product value for coronary artery disease is 98 % to 99 % .
	manualset3
224389	1	420944	7	NULL	NULL	0	NULL	habit	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As the habit is stabilized , the number of interhemispheric correlations increases , which testifies to the enhancement of the paired function of the cerebral hemispheres .
	manualset3
224390	2	420944	7	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	As the habit is stabilized , the number of interhemispheric correlations increases , which testifies to the enhancement of the paired function of the cerebral hemispheres .
	manualset3
224391	3	420944	7	NULL	NULL	0	NULL	interhemispheric correlations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	As the habit is stabilized , the number of interhemispheric correlations increases , which testifies to the enhancement of the paired function of the cerebral hemispheres .
	manualset3
224392	4	420944	7	NULL	NULL	0	NULL	enhancement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As the habit is stabilized , the number of interhemispheric correlations increases , which testifies to the enhancement of the paired function of the cerebral hemispheres .
	manualset3
224393	5	420944	7	NULL	NULL	0	NULL	 paired function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As the habit is stabilized , the number of interhemispheric correlations increases , which testifies to the enhancement of the paired function of the cerebral hemispheres .
	manualset3
224394	6	420944	7	NULL	NULL	0	NULL	 cerebral hemispheres	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	As the habit is stabilized , the number of interhemispheric correlations increases , which testifies to the enhancement of the paired function of the cerebral hemispheres .
	manualset3
224395	1	420945	7	NULL	NULL	0	NULL	one device	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Only one device , based on reverse osmosis , was capable of removing F-RNA phages at concentrations under the detection limit and microcystins by 2.5 log10 .
	manualset3
224396	2	420945	7	NULL	NULL	0	NULL	reverse osmosis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Only one device , based on reverse osmosis , was capable of removing F-RNA phages at concentrations under the detection limit and microcystins by 2.5 log10 .
	manualset3
224397	3	420945	7	NULL	NULL	NULL	NULL	removing	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Only one device , based on reverse osmosis , was capable of removing F-RNA phages at concentrations under the detection limit and microcystins by 2.5 log10 .
	manualset3
224398	4	420945	7	NULL	NULL	0	NULL	F-RNA phages 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Only one device , based on reverse osmosis , was capable of removing F-RNA phages at concentrations under the detection limit and microcystins by 2.5 log10 .
	manualset3
224399	5	420945	7	NULL	NULL	0	NULL	concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Only one device , based on reverse osmosis , was capable of removing F-RNA phages at concentrations under the detection limit and microcystins by 2.5 log10 .
	manualset3
224400	6	420945	7	NULL	NULL	0	NULL	detection limit 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Only one device , based on reverse osmosis , was capable of removing F-RNA phages at concentrations under the detection limit and microcystins by 2.5 log10 .
	manualset3
224401	7	420945	7	NULL	NULL	0	NULL	microcystins	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Only one device , based on reverse osmosis , was capable of removing F-RNA phages at concentrations under the detection limit and microcystins by 2.5 log10 .
	manualset3
224402	8	420945	7	NULL	NULL	0	NULL	2.5 log10	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Only one device , based on reverse osmosis , was capable of removing F-RNA phages at concentrations under the detection limit and microcystins by 2.5 log10 .
	manualset3
224403	1	420946	7	NULL	NULL	0	NULL	two analogs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The two analogs are : Nalpha-Methyl-Tyrosyl-Glycyl-Glycyl-Phenylalanyl-des-carboxy-Norleucine ( I ) and Tyrosyl-D-Alanyl-Glycyl-Phenylalanyl-des-carboxy-Norleucine ( II ) .
	manualset3
224404	2	420946	7	NULL	NULL	0	NULL	Nalpha-Methyl-Tyrosyl-Glycyl-Glycyl-Phenylalanyl-des-carboxy-Norleucine ( I )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The two analogs are : Nalpha-Methyl-Tyrosyl-Glycyl-Glycyl-Phenylalanyl-des-carboxy-Norleucine ( I ) and Tyrosyl-D-Alanyl-Glycyl-Phenylalanyl-des-carboxy-Norleucine ( II ) .
	manualset3
224405	3	420946	7	NULL	NULL	0	NULL	Tyrosyl-D-Alanyl-Glycyl-Phenylalanyl-des-carboxy-Norleucine ( II )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The two analogs are : Nalpha-Methyl-Tyrosyl-Glycyl-Glycyl-Phenylalanyl-des-carboxy-Norleucine ( I ) and Tyrosyl-D-Alanyl-Glycyl-Phenylalanyl-des-carboxy-Norleucine ( II ) .
	manualset3
224406	1	420947	7	NULL	NULL	0	NULL	Patient feedback	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient feedback has shown the sessions meet their needs and staff have found that less time is taken up during individual appointments answering commonly asked questions and repeating information that is frequently asked for .
	manualset3
224407	2	420947	7	NULL	NULL	0	NULL	sessions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient feedback has shown the sessions meet their needs and staff have found that less time is taken up during individual appointments answering commonly asked questions and repeating information that is frequently asked for .
	manualset3
224408	3	420947	7	NULL	NULL	0	NULL	needs 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient feedback has shown the sessions meet their needs and staff have found that less time is taken up during individual appointments answering commonly asked questions and repeating information that is frequently asked for .
	manualset3
224409	4	420947	7	NULL	NULL	0	NULL	staff 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient feedback has shown the sessions meet their needs and staff have found that less time is taken up during individual appointments answering commonly asked questions and repeating information that is frequently asked for .
	manualset3
224410	5	420947	7	NULL	NULL	0	NULL	less time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient feedback has shown the sessions meet their needs and staff have found that less time is taken up during individual appointments answering commonly asked questions and repeating information that is frequently asked for .
	manualset3
224411	6	420947	7	NULL	NULL	0	NULL	individual appointments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient feedback has shown the sessions meet their needs and staff have found that less time is taken up during individual appointments answering commonly asked questions and repeating information that is frequently asked for .
	manualset3
224412	7	420947	7	NULL	NULL	0	NULL	commonly asked questions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Patient feedback has shown the sessions meet their needs and staff have found that less time is taken up during individual appointments answering commonly asked questions and repeating information that is frequently asked for .
	manualset3
224413	8	420947	7	NULL	NULL	NULL	NULL	repeating information	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Patient feedback has shown the sessions meet their needs and staff have found that less time is taken up during individual appointments answering commonly asked questions and repeating information that is frequently asked for .
	manualset3
224415	1	420948	7	NULL	NULL	0	NULL	extrahypothalamic brain regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the extrahypothalamic brain regions examined , the levels of cyclo ( His-Pro ) were highest in the cerebellar hemisphere ( 0.168 ng/mg protein ) and olfactory bulbs ( 0.180 ng/mg protein ) and were lowest in the hippocampus ( 0.080 ng/mg protein ) and occipital cortex ( 0.079 ng/mg protein ) .
	manualset3
224416	2	420948	7	NULL	NULL	0	NULL	levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the extrahypothalamic brain regions examined , the levels of cyclo ( His-Pro ) were highest in the cerebellar hemisphere ( 0.168 ng/mg protein ) and olfactory bulbs ( 0.180 ng/mg protein ) and were lowest in the hippocampus ( 0.080 ng/mg protein ) and occipital cortex ( 0.079 ng/mg protein ) .
	manualset3
224417	3	420948	7	NULL	NULL	0	NULL	cyclo ( His-Pro )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the extrahypothalamic brain regions examined , the levels of cyclo ( His-Pro ) were highest in the cerebellar hemisphere ( 0.168 ng/mg protein ) and olfactory bulbs ( 0.180 ng/mg protein ) and were lowest in the hippocampus ( 0.080 ng/mg protein ) and occipital cortex ( 0.079 ng/mg protein ) .
	manualset3
224418	4	420948	7	NULL	NULL	0	NULL	cerebellar hemisphere 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the extrahypothalamic brain regions examined , the levels of cyclo ( His-Pro ) were highest in the cerebellar hemisphere ( 0.168 ng/mg protein ) and olfactory bulbs ( 0.180 ng/mg protein ) and were lowest in the hippocampus ( 0.080 ng/mg protein ) and occipital cortex ( 0.079 ng/mg protein ) .
	manualset3
224419	5	420948	7	NULL	NULL	0	NULL	0.168 ng/mg protein	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the extrahypothalamic brain regions examined , the levels of cyclo ( His-Pro ) were highest in the cerebellar hemisphere ( 0.168 ng/mg protein ) and olfactory bulbs ( 0.180 ng/mg protein ) and were lowest in the hippocampus ( 0.080 ng/mg protein ) and occipital cortex ( 0.079 ng/mg protein ) .
	manualset3
224420	6	420948	7	NULL	NULL	0	NULL	olfactory bulbs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the extrahypothalamic brain regions examined , the levels of cyclo ( His-Pro ) were highest in the cerebellar hemisphere ( 0.168 ng/mg protein ) and olfactory bulbs ( 0.180 ng/mg protein ) and were lowest in the hippocampus ( 0.080 ng/mg protein ) and occipital cortex ( 0.079 ng/mg protein ) .
	manualset3
224421	7	420948	7	NULL	NULL	NULL	NULL	0.180 ng/mg protein	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Among the extrahypothalamic brain regions examined , the levels of cyclo ( His-Pro ) were highest in the cerebellar hemisphere ( 0.168 ng/mg protein ) and olfactory bulbs ( 0.180 ng/mg protein ) and were lowest in the hippocampus ( 0.080 ng/mg protein ) and occipital cortex ( 0.079 ng/mg protein ) .
	manualset3
224422	8	420948	7	NULL	NULL	0	NULL	hippocampus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the extrahypothalamic brain regions examined , the levels of cyclo ( His-Pro ) were highest in the cerebellar hemisphere ( 0.168 ng/mg protein ) and olfactory bulbs ( 0.180 ng/mg protein ) and were lowest in the hippocampus ( 0.080 ng/mg protein ) and occipital cortex ( 0.079 ng/mg protein ) .
	manualset3
224423	9	420948	7	NULL	NULL	0	NULL	 0.080 ng/mg protein	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the extrahypothalamic brain regions examined , the levels of cyclo ( His-Pro ) were highest in the cerebellar hemisphere ( 0.168 ng/mg protein ) and olfactory bulbs ( 0.180 ng/mg protein ) and were lowest in the hippocampus ( 0.080 ng/mg protein ) and occipital cortex ( 0.079 ng/mg protein ) .
	manualset3
224424	10	420948	7	NULL	NULL	0	NULL	occipital cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the extrahypothalamic brain regions examined , the levels of cyclo ( His-Pro ) were highest in the cerebellar hemisphere ( 0.168 ng/mg protein ) and olfactory bulbs ( 0.180 ng/mg protein ) and were lowest in the hippocampus ( 0.080 ng/mg protein ) and occipital cortex ( 0.079 ng/mg protein ) .
	manualset3
224425	11	420948	7	NULL	NULL	0	NULL	0.079 ng/mg protein	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the extrahypothalamic brain regions examined , the levels of cyclo ( His-Pro ) were highest in the cerebellar hemisphere ( 0.168 ng/mg protein ) and olfactory bulbs ( 0.180 ng/mg protein ) and were lowest in the hippocampus ( 0.080 ng/mg protein ) and occipital cortex ( 0.079 ng/mg protein ) .
	manualset3
224426	1	420949	7	NULL	NULL	0	NULL	vIL-10 probe detected transcripts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The vIL-10 probe detected transcripts in lytically infected cell lines and within the differentiated layers of oral hairy leukoplakia .
	manualset3
224427	2	420949	7	NULL	NULL	0	NULL	lytically infected cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The vIL-10 probe detected transcripts in lytically infected cell lines and within the differentiated layers of oral hairy leukoplakia .
	manualset3
224428	3	420949	7	NULL	NULL	0	NULL	differentiated layers	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The vIL-10 probe detected transcripts in lytically infected cell lines and within the differentiated layers of oral hairy leukoplakia .
	manualset3
224429	4	420949	7	NULL	NULL	0	NULL	oral hairy leukoplakia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The vIL-10 probe detected transcripts in lytically infected cell lines and within the differentiated layers of oral hairy leukoplakia .
	manualset3
224430	1	420950	7	NULL	NULL	NULL	NULL	Graduate medical education reform	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Graduate medical education reform : implications for emergency medicine resident training .
	manualset3
224431	2	420950	7	NULL	NULL	0	NULL	implications 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Graduate medical education reform : implications for emergency medicine resident training .
	manualset3
224432	3	420950	7	NULL	NULL	0	NULL	emergency medicine resident training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Graduate medical education reform : implications for emergency medicine resident training .
	manualset3
224433	1	420951	7	NULL	NULL	0	NULL	Cue interactions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Cue interactions in flavor preference learning : a configural analysis .
	manualset3
224434	2	420951	7	NULL	NULL	NULL	NULL	flavor preference learning	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cue interactions in flavor preference learning : a configural analysis .
	manualset3
224435	3	420951	7	NULL	NULL	0	NULL	configural analysis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Cue interactions in flavor preference learning : a configural analysis .
	manualset3
224436	1	420952	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results agree with previous studies suggesting that adaptation requires positive selection , but not every mutation under positive selection contributes to the adaptive dynamical process of the evolution of species .
	manualset3
224437	2	420952	7	NULL	NULL	0	NULL	previous studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results agree with previous studies suggesting that adaptation requires positive selection , but not every mutation under positive selection contributes to the adaptive dynamical process of the evolution of species .
	manualset3
224438	3	420952	7	NULL	NULL	0	NULL	adaptation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results agree with previous studies suggesting that adaptation requires positive selection , but not every mutation under positive selection contributes to the adaptive dynamical process of the evolution of species .
	manualset3
224439	4	420952	7	NULL	NULL	0	NULL	positive selection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results agree with previous studies suggesting that adaptation requires positive selection , but not every mutation under positive selection contributes to the adaptive dynamical process of the evolution of species .
	manualset3
224440	5	420952	7	NULL	NULL	0	NULL	mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results agree with previous studies suggesting that adaptation requires positive selection , but not every mutation under positive selection contributes to the adaptive dynamical process of the evolution of species .
	manualset3
224441	6	420952	7	NULL	NULL	0	NULL	positive selection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results agree with previous studies suggesting that adaptation requires positive selection , but not every mutation under positive selection contributes to the adaptive dynamical process of the evolution of species .
	manualset3
224442	7	420952	7	NULL	NULL	0	NULL	adaptive dynamical process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results agree with previous studies suggesting that adaptation requires positive selection , but not every mutation under positive selection contributes to the adaptive dynamical process of the evolution of species .
	manualset3
224443	8	420952	7	NULL	NULL	0	NULL	evolution 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results agree with previous studies suggesting that adaptation requires positive selection , but not every mutation under positive selection contributes to the adaptive dynamical process of the evolution of species .
	manualset3
224444	9	420952	7	NULL	NULL	0	NULL	species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results agree with previous studies suggesting that adaptation requires positive selection , but not every mutation under positive selection contributes to the adaptive dynamical process of the evolution of species .
	manualset3
224445	1	420953	7	NULL	NULL	0	NULL	Failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Failure to detect surfactant protein-specific antibodies in sera of premature infants treated with survanta , a modified bovine surfactant .
	manualset3
224446	2	420953	7	NULL	NULL	0	NULL	surfactant protein-specific antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Failure to detect surfactant protein-specific antibodies in sera of premature infants treated with survanta , a modified bovine surfactant .
	manualset3
224447	3	420953	7	NULL	NULL	0	NULL	sera 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Failure to detect surfactant protein-specific antibodies in sera of premature infants treated with survanta , a modified bovine surfactant .
	manualset3
224448	4	420953	7	NULL	NULL	0	NULL	premature infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Failure to detect surfactant protein-specific antibodies in sera of premature infants treated with survanta , a modified bovine surfactant .
	manualset3
224449	5	420953	7	NULL	NULL	0	NULL	survanta	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Failure to detect surfactant protein-specific antibodies in sera of premature infants treated with survanta , a modified bovine surfactant .
	manualset3
224450	6	420953	7	NULL	NULL	0	NULL	modified bovine surfactant	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Failure to detect surfactant protein-specific antibodies in sera of premature infants treated with survanta , a modified bovine surfactant .
	manualset3
224451	1	420954	7	NULL	NULL	0	NULL	Examples 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Examples of questions include : `` Do you use drugs mostly to make bad feelings like boredom , loneliness , or apathy go away ? ''
	manualset3
224452	2	420954	7	NULL	NULL	0	NULL	questions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Examples of questions include : `` Do you use drugs mostly to make bad feelings like boredom , loneliness , or apathy go away ? ''
	manualset3
224453	3	420954	7	NULL	NULL	0	NULL	 drugs 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Examples of questions include : `` Do you use drugs mostly to make bad feelings like boredom , loneliness , or apathy go away ? ''
	manualset3
224454	4	420954	7	NULL	NULL	0	NULL	bad feelings	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Examples of questions include : `` Do you use drugs mostly to make bad feelings like boredom , loneliness , or apathy go away ? ''
	manualset3
224455	5	420954	7	NULL	NULL	0	NULL	boredom	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Examples of questions include : `` Do you use drugs mostly to make bad feelings like boredom , loneliness , or apathy go away ? ''
	manualset3
224456	6	420954	7	NULL	NULL	0	NULL	 loneliness	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Examples of questions include : `` Do you use drugs mostly to make bad feelings like boredom , loneliness , or apathy go away ? ''
	manualset3
224457	7	420954	7	NULL	NULL	0	NULL	apathy	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Examples of questions include : `` Do you use drugs mostly to make bad feelings like boredom , loneliness , or apathy go away ? ''
	manualset3
224458	1	420955	7	NULL	NULL	0	NULL	Observations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Observations on cysteic acid decarboxylase .
	manualset3
224459	2	420955	7	NULL	NULL	0	NULL	cysteic acid decarboxylase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Observations on cysteic acid decarboxylase .
	manualset3
224460	1	420956	7	NULL	NULL	0	NULL	imported diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the imported diseases , malaria , typhoid and tuberculosis should always be considered in cases of fever .
	manualset3
224461	2	420956	7	NULL	NULL	0	NULL	malaria	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the imported diseases , malaria , typhoid and tuberculosis should always be considered in cases of fever .
	manualset3
224462	3	420956	7	NULL	NULL	0	NULL	typhoid	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the imported diseases , malaria , typhoid and tuberculosis should always be considered in cases of fever .
	manualset3
224463	4	420956	7	NULL	NULL	0	NULL	 tuberculosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the imported diseases , malaria , typhoid and tuberculosis should always be considered in cases of fever .
	manualset3
224464	5	420956	7	NULL	NULL	0	NULL	cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the imported diseases , malaria , typhoid and tuberculosis should always be considered in cases of fever .
	manualset3
224465	6	420956	7	NULL	NULL	0	NULL	fever	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the imported diseases , malaria , typhoid and tuberculosis should always be considered in cases of fever .
	manualset3
224466	1	420957	7	NULL	NULL	0	NULL	human lymphoblastoid cell line 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
224467	2	420957	7	NULL	NULL	0	NULL	gamma irradiation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
224468	3	420957	7	NULL	NULL	0	NULL	0.5 Gy	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
224469	4	420957	7	NULL	NULL	0	NULL	1 Gy	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
224470	5	420957	7	NULL	NULL	0	NULL	2 Gy	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
224471	6	420957	7	NULL	NULL	0	NULL	4 Gy	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
224472	7	420957	7	NULL	NULL	0	NULL	8 Gy	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
224473	8	420957	7	NULL	NULL	0	NULL	 16 Gy	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
224474	9	420957	7	NULL	NULL	0	NULL	16 Gy	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
224475	10	420957	7	NULL	NULL	0	NULL	32 Gy	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
224476	11	420957	7	NULL	NULL	0	NULL	0.5 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
224477	12	420957	7	NULL	NULL	0	NULL	24 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
224478	13	420957	7	NULL	NULL	0	NULL	 48 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
224479	14	420957	7	NULL	NULL	0	NULL	72 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
224480	15	420957	7	NULL	NULL	0	NULL	 treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
224481	16	420957	7	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
224482	17	420957	7	NULL	NULL	0	NULL	proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
224483	18	420957	7	NULL	NULL	0	NULL	cell cycle analysis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
224484	19	420957	7	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
224485	20	420957	7	NULL	NULL	0	NULL	micronuclei frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
224486	21	420957	7	NULL	NULL	0	NULL	 expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
224487	22	420957	7	NULL	NULL	0	NULL	TP53	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
224488	23	420957	7	NULL	NULL	0	NULL	WAF1	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
224489	24	420957	7	NULL	NULL	NULL	NULL	DNA LIGASE 1 	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
224490	25	420957	7	NULL	NULL	0	NULL	BAX	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
224491	26	420957	7	NULL	NULL	0	NULL	BLC-2	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
224492	27	420957	7	NULL	NULL	0	NULL	BAK 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
224493	28	420957	7	NULL	NULL	0	NULL	DAD1	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
224494	29	420957	7	NULL	NULL	0	NULL	 ICH1-Long mRNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
224495	30	420957	7	NULL	NULL	0	NULL	 ICH1-Short forms mRNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
226671	31	420957	7	NULL	NULL	0	NULL	PCNA	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a human lymphoblastoid cell line , we have analyzed , following gamma irradiation ( 0.5 , 1 , 2 , 4 , 8 , 16 and 32 Gy , at 0.5 , 24 , 48 and 72 h after treatment ) , the correlation between proliferation , cell cycle analysis , apoptosis and micronuclei frequency with the expression of TP53 , WAF1 , DNA LIGASE 1 , PCNA , BAX , BLC-2 , BAK , DAD1 , ICH1-Long and - Short forms mRNAs .
	manualset3
224496	1	420958	7	NULL	NULL	0	NULL	1 hr 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 1 hr after addition of serum , there was also an increase in the level of a nuclear protein that bound to the two CCAAT boxes , even in the presence of cycloheximide .
	manualset3
224497	2	420958	7	NULL	NULL	0	NULL	serum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 1 hr after addition of serum , there was also an increase in the level of a nuclear protein that bound to the two CCAAT boxes , even in the presence of cycloheximide .
	manualset3
224498	3	420958	7	NULL	NULL	0	NULL	level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 1 hr after addition of serum , there was also an increase in the level of a nuclear protein that bound to the two CCAAT boxes , even in the presence of cycloheximide .
	manualset3
224499	4	420958	7	NULL	NULL	0	NULL	nuclear protein 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 1 hr after addition of serum , there was also an increase in the level of a nuclear protein that bound to the two CCAAT boxes , even in the presence of cycloheximide .
	manualset3
224500	5	420958	7	NULL	NULL	0	NULL	 two CCAAT boxes	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 1 hr after addition of serum , there was also an increase in the level of a nuclear protein that bound to the two CCAAT boxes , even in the presence of cycloheximide .
	manualset3
224501	6	420958	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 1 hr after addition of serum , there was also an increase in the level of a nuclear protein that bound to the two CCAAT boxes , even in the presence of cycloheximide .
	manualset3
224502	7	420958	7	NULL	NULL	0	NULL	cycloheximide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 1 hr after addition of serum , there was also an increase in the level of a nuclear protein that bound to the two CCAAT boxes , even in the presence of cycloheximide .
	manualset3
224503	8	420958	7	NULL	NULL	0	NULL	increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 1 hr after addition of serum , there was also an increase in the level of a nuclear protein that bound to the two CCAAT boxes , even in the presence of cycloheximide .
	manualset3
224504	9	420958	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Within 1 hr after addition of serum , there was also an increase in the level of a nuclear protein that bound to the two CCAAT boxes , even in the presence of cycloheximide .
	manualset3
224505	1	420959	7	NULL	NULL	0	NULL	low-numerical-aperture ( NA ) OCT system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	While a low-numerical-aperture ( NA ) OCT system can tolerate defocus because the depth of field is large , for high NA it is critical to correct for defocus .
	manualset3
224506	2	420959	7	NULL	NULL	0	NULL	defocus	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While a low-numerical-aperture ( NA ) OCT system can tolerate defocus because the depth of field is large , for high NA it is critical to correct for defocus .
	manualset3
224507	3	420959	7	NULL	NULL	0	NULL	depth of field	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While a low-numerical-aperture ( NA ) OCT system can tolerate defocus because the depth of field is large , for high NA it is critical to correct for defocus .
	manualset3
224508	4	420959	7	NULL	NULL	0	NULL	 high NA	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	While a low-numerical-aperture ( NA ) OCT system can tolerate defocus because the depth of field is large , for high NA it is critical to correct for defocus .
	manualset3
224509	5	420959	7	NULL	NULL	0	NULL	defocus	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	While a low-numerical-aperture ( NA ) OCT system can tolerate defocus because the depth of field is large , for high NA it is critical to correct for defocus .
	manualset3
224510	1	420960	7	NULL	NULL	0	NULL	novel interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel interaction between human DNA polymerase eta and MutLalpha .
	manualset3
224511	2	420960	7	NULL	NULL	0	NULL	human DNA polymerase eta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel interaction between human DNA polymerase eta and MutLalpha .
	manualset3
224512	3	420960	7	NULL	NULL	0	NULL	MutLalpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel interaction between human DNA polymerase eta and MutLalpha .
	manualset3
224513	1	420961	7	NULL	NULL	0	NULL	Haemophilus influenzae type b vaccine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The Haemophilus influenzae type b vaccine ( HibTITER ) given concurrently in the contralateral site to the pertussis vaccine showed the same lower rates in both studies for ventrogluteal injection compared with anterolateral thigh injection for local reactions ( redness/swelling both studies ( P & lt ; 0.0001 ) and bruising DTPw study ( P & lt ; 0.0001 ) and DTPa study ( P & lt ; 0.0004 ) ) .
	manualset3
224514	2	420961	7	NULL	NULL	0	NULL	HibTITER	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Haemophilus influenzae type b vaccine ( HibTITER ) given concurrently in the contralateral site to the pertussis vaccine showed the same lower rates in both studies for ventrogluteal injection compared with anterolateral thigh injection for local reactions ( redness/swelling both studies ( P & lt ; 0.0001 ) and bruising DTPw study ( P & lt ; 0.0001 ) and DTPa study ( P & lt ; 0.0004 ) ) .
	manualset3
224515	3	420961	7	NULL	NULL	0	NULL	contralateral site	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The Haemophilus influenzae type b vaccine ( HibTITER ) given concurrently in the contralateral site to the pertussis vaccine showed the same lower rates in both studies for ventrogluteal injection compared with anterolateral thigh injection for local reactions ( redness/swelling both studies ( P & lt ; 0.0001 ) and bruising DTPw study ( P & lt ; 0.0001 ) and DTPa study ( P & lt ; 0.0004 ) ) .
	manualset3
224516	4	420961	7	NULL	NULL	0	NULL	pertussis vaccine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The Haemophilus influenzae type b vaccine ( HibTITER ) given concurrently in the contralateral site to the pertussis vaccine showed the same lower rates in both studies for ventrogluteal injection compared with anterolateral thigh injection for local reactions ( redness/swelling both studies ( P & lt ; 0.0001 ) and bruising DTPw study ( P & lt ; 0.0001 ) and DTPa study ( P & lt ; 0.0004 ) ) .
	manualset3
224517	5	420961	7	NULL	NULL	0	NULL	lower rates 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Haemophilus influenzae type b vaccine ( HibTITER ) given concurrently in the contralateral site to the pertussis vaccine showed the same lower rates in both studies for ventrogluteal injection compared with anterolateral thigh injection for local reactions ( redness/swelling both studies ( P & lt ; 0.0001 ) and bruising DTPw study ( P & lt ; 0.0001 ) and DTPa study ( P & lt ; 0.0004 ) ) .
	manualset3
224518	6	420961	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Haemophilus influenzae type b vaccine ( HibTITER ) given concurrently in the contralateral site to the pertussis vaccine showed the same lower rates in both studies for ventrogluteal injection compared with anterolateral thigh injection for local reactions ( redness/swelling both studies ( P & lt ; 0.0001 ) and bruising DTPw study ( P & lt ; 0.0001 ) and DTPa study ( P & lt ; 0.0004 ) ) .
	manualset3
224519	7	420961	7	NULL	NULL	0	NULL	ventrogluteal injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The Haemophilus influenzae type b vaccine ( HibTITER ) given concurrently in the contralateral site to the pertussis vaccine showed the same lower rates in both studies for ventrogluteal injection compared with anterolateral thigh injection for local reactions ( redness/swelling both studies ( P & lt ; 0.0001 ) and bruising DTPw study ( P & lt ; 0.0001 ) and DTPa study ( P & lt ; 0.0004 ) ) .
	manualset3
224520	8	420961	7	NULL	NULL	0	NULL	anterolateral thigh injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The Haemophilus influenzae type b vaccine ( HibTITER ) given concurrently in the contralateral site to the pertussis vaccine showed the same lower rates in both studies for ventrogluteal injection compared with anterolateral thigh injection for local reactions ( redness/swelling both studies ( P & lt ; 0.0001 ) and bruising DTPw study ( P & lt ; 0.0001 ) and DTPa study ( P & lt ; 0.0004 ) ) .
	manualset3
224521	9	420961	7	NULL	NULL	0	NULL	local reactions 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Haemophilus influenzae type b vaccine ( HibTITER ) given concurrently in the contralateral site to the pertussis vaccine showed the same lower rates in both studies for ventrogluteal injection compared with anterolateral thigh injection for local reactions ( redness/swelling both studies ( P & lt ; 0.0001 ) and bruising DTPw study ( P & lt ; 0.0001 ) and DTPa study ( P & lt ; 0.0004 ) ) .
	manualset3
224522	10	420961	7	NULL	NULL	0	NULL	redness/swelling	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The Haemophilus influenzae type b vaccine ( HibTITER ) given concurrently in the contralateral site to the pertussis vaccine showed the same lower rates in both studies for ventrogluteal injection compared with anterolateral thigh injection for local reactions ( redness/swelling both studies ( P & lt ; 0.0001 ) and bruising DTPw study ( P & lt ; 0.0001 ) and DTPa study ( P & lt ; 0.0004 ) ) .
	manualset3
224523	11	420961	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Haemophilus influenzae type b vaccine ( HibTITER ) given concurrently in the contralateral site to the pertussis vaccine showed the same lower rates in both studies for ventrogluteal injection compared with anterolateral thigh injection for local reactions ( redness/swelling both studies ( P & lt ; 0.0001 ) and bruising DTPw study ( P & lt ; 0.0001 ) and DTPa study ( P & lt ; 0.0004 ) ) .
	manualset3
224524	12	420961	7	NULL	NULL	0	NULL	P & lt ; 0.0001	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Haemophilus influenzae type b vaccine ( HibTITER ) given concurrently in the contralateral site to the pertussis vaccine showed the same lower rates in both studies for ventrogluteal injection compared with anterolateral thigh injection for local reactions ( redness/swelling both studies ( P & lt ; 0.0001 ) and bruising DTPw study ( P & lt ; 0.0001 ) and DTPa study ( P & lt ; 0.0004 ) ) .
	manualset3
224525	13	420961	7	NULL	NULL	0	NULL	DTPw study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Haemophilus influenzae type b vaccine ( HibTITER ) given concurrently in the contralateral site to the pertussis vaccine showed the same lower rates in both studies for ventrogluteal injection compared with anterolateral thigh injection for local reactions ( redness/swelling both studies ( P & lt ; 0.0001 ) and bruising DTPw study ( P & lt ; 0.0001 ) and DTPa study ( P & lt ; 0.0004 ) ) .
	manualset3
224526	14	420961	7	NULL	NULL	0	NULL	P & lt ; 0.0001 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Haemophilus influenzae type b vaccine ( HibTITER ) given concurrently in the contralateral site to the pertussis vaccine showed the same lower rates in both studies for ventrogluteal injection compared with anterolateral thigh injection for local reactions ( redness/swelling both studies ( P & lt ; 0.0001 ) and bruising DTPw study ( P & lt ; 0.0001 ) and DTPa study ( P & lt ; 0.0004 ) ) .
	manualset3
224527	15	420961	7	NULL	NULL	0	NULL	DTPa study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Haemophilus influenzae type b vaccine ( HibTITER ) given concurrently in the contralateral site to the pertussis vaccine showed the same lower rates in both studies for ventrogluteal injection compared with anterolateral thigh injection for local reactions ( redness/swelling both studies ( P & lt ; 0.0001 ) and bruising DTPw study ( P & lt ; 0.0001 ) and DTPa study ( P & lt ; 0.0004 ) ) .
	manualset3
224528	16	420961	7	NULL	NULL	0	NULL	P & lt ; 0.0004	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The Haemophilus influenzae type b vaccine ( HibTITER ) given concurrently in the contralateral site to the pertussis vaccine showed the same lower rates in both studies for ventrogluteal injection compared with anterolateral thigh injection for local reactions ( redness/swelling both studies ( P & lt ; 0.0001 ) and bruising DTPw study ( P & lt ; 0.0001 ) and DTPa study ( P & lt ; 0.0004 ) ) .
	manualset3
224529	1	420962	7	NULL	NULL	0	NULL	Clinical evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical evaluation of the diagnosis of neuronal reversibility with acute cerebral infarction using ADC by diffusion weighted echo planar imaging ) .
	manualset3
224530	2	420962	7	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical evaluation of the diagnosis of neuronal reversibility with acute cerebral infarction using ADC by diffusion weighted echo planar imaging ) .
	manualset3
224531	3	420962	7	NULL	NULL	0	NULL	neuronal reversibility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical evaluation of the diagnosis of neuronal reversibility with acute cerebral infarction using ADC by diffusion weighted echo planar imaging ) .
	manualset3
224532	4	420962	7	NULL	NULL	0	NULL	acute cerebral infarction 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical evaluation of the diagnosis of neuronal reversibility with acute cerebral infarction using ADC by diffusion weighted echo planar imaging ) .
	manualset3
224533	5	420962	7	NULL	NULL	0	NULL	 ADC	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical evaluation of the diagnosis of neuronal reversibility with acute cerebral infarction using ADC by diffusion weighted echo planar imaging ) .
	manualset3
224534	6	420962	7	NULL	NULL	0	NULL	diffusion weighted echo planar imaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical evaluation of the diagnosis of neuronal reversibility with acute cerebral infarction using ADC by diffusion weighted echo planar imaging ) .
	manualset3
224535	1	420963	7	NULL	NULL	0	NULL	retrospective chart review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	We attempted to do this with a retrospective chart review of 188 bipolar patients seen by D.L. Dunner between January 1992 and December 1993 .
	manualset3
224536	2	420963	7	NULL	NULL	0	NULL	188 bipolar patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We attempted to do this with a retrospective chart review of 188 bipolar patients seen by D.L. Dunner between January 1992 and December 1993 .
	manualset3
224537	3	420963	7	NULL	NULL	0	NULL	D.L. Dunner 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	We attempted to do this with a retrospective chart review of 188 bipolar patients seen by D.L. Dunner between January 1992 and December 1993 .
	manualset3
224538	4	420963	7	NULL	NULL	0	NULL	January 1992	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	We attempted to do this with a retrospective chart review of 188 bipolar patients seen by D.L. Dunner between January 1992 and December 1993 .
	manualset3
224539	5	420963	7	NULL	NULL	0	NULL	December 1993	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	We attempted to do this with a retrospective chart review of 188 bipolar patients seen by D.L. Dunner between January 1992 and December 1993 .
	manualset3
224540	1	420964	7	NULL	NULL	0	NULL	activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the most characterized activities of Tau is the ability to regulate microtubule dynamics , known to be essential for proper cell function and viability .
	manualset3
224541	2	420964	7	NULL	NULL	0	NULL	Tau	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the most characterized activities of Tau is the ability to regulate microtubule dynamics , known to be essential for proper cell function and viability .
	manualset3
224542	3	420964	7	NULL	NULL	0	NULL	microtubule dynamics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the most characterized activities of Tau is the ability to regulate microtubule dynamics , known to be essential for proper cell function and viability .
	manualset3
224543	4	420964	7	NULL	NULL	0	NULL	cell function 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the most characterized activities of Tau is the ability to regulate microtubule dynamics , known to be essential for proper cell function and viability .
	manualset3
224544	5	420964	7	NULL	NULL	0	NULL	 viability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the most characterized activities of Tau is the ability to regulate microtubule dynamics , known to be essential for proper cell function and viability .
	manualset3
226672	6	420964	7	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the most characterized activities of Tau is the ability to regulate microtubule dynamics , known to be essential for proper cell function and viability .
	manualset3
224545	1	420965	7	NULL	NULL	0	NULL	Cost-effectiveness analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Cost-effectiveness analysis of flexible optical scopes for tracheal intubation : a descriptive comparative study of reusable and single-use scopes .
	manualset3
224546	2	420965	7	NULL	NULL	NULL	NULL	flexible optical scopes	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cost-effectiveness analysis of flexible optical scopes for tracheal intubation : a descriptive comparative study of reusable and single-use scopes .
	manualset3
224547	3	420965	7	NULL	NULL	0	NULL	tracheal intubation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Cost-effectiveness analysis of flexible optical scopes for tracheal intubation : a descriptive comparative study of reusable and single-use scopes .
	manualset3
224548	4	420965	7	NULL	NULL	0	NULL	descriptive comparative study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Cost-effectiveness analysis of flexible optical scopes for tracheal intubation : a descriptive comparative study of reusable and single-use scopes .
	manualset3
224549	5	420965	7	NULL	NULL	0	NULL	reusable scopes	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Cost-effectiveness analysis of flexible optical scopes for tracheal intubation : a descriptive comparative study of reusable and single-use scopes .
	manualset3
224550	6	420965	7	NULL	NULL	0	NULL	single-use scopes	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Cost-effectiveness analysis of flexible optical scopes for tracheal intubation : a descriptive comparative study of reusable and single-use scopes .
	manualset3
224551	1	420966	7	NULL	NULL	0	NULL	Recent advances 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in avian biochemistry : the fatty liver and kidney syndrome .
	manualset3
224552	2	420966	7	NULL	NULL	0	NULL	avian biochemistry	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in avian biochemistry : the fatty liver and kidney syndrome .
	manualset3
224553	3	420966	7	NULL	NULL	0	NULL	fatty liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in avian biochemistry : the fatty liver and kidney syndrome .
	manualset3
224554	4	420966	7	NULL	NULL	0	NULL	kidney syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent advances in avian biochemistry : the fatty liver and kidney syndrome .
	manualset3
224555	1	420967	7	NULL	NULL	0	NULL	Serotonin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Serotonin , PGE2 and PGF2 alpha caused biphasic responses in which both the dilator and the constrictor phases were found to be dose-dependent .
	manualset3
224556	2	420967	7	NULL	NULL	0	NULL	PGE2	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Serotonin , PGE2 and PGF2 alpha caused biphasic responses in which both the dilator and the constrictor phases were found to be dose-dependent .
	manualset3
224557	3	420967	7	NULL	NULL	0	NULL	PGF2 alpha	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Serotonin , PGE2 and PGF2 alpha caused biphasic responses in which both the dilator and the constrictor phases were found to be dose-dependent .
	manualset3
224558	4	420967	7	NULL	NULL	0	NULL	biphasic responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serotonin , PGE2 and PGF2 alpha caused biphasic responses in which both the dilator and the constrictor phases were found to be dose-dependent .
	manualset3
224559	5	420967	7	NULL	NULL	0	NULL	dilator phases	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Serotonin , PGE2 and PGF2 alpha caused biphasic responses in which both the dilator and the constrictor phases were found to be dose-dependent .
	manualset3
224560	6	420967	7	NULL	NULL	0	NULL	constrictor phases	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Serotonin , PGE2 and PGF2 alpha caused biphasic responses in which both the dilator and the constrictor phases were found to be dose-dependent .
	manualset3
224561	1	420968	7	NULL	NULL	0	NULL	Feed conversion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Feed conversion ( P & lt ; 0.01 ) and egg production ( P & lt ; 0.01 ) improved most when both zinc and pyridoxine were supplemented to the diet .
	manualset3
224562	2	420968	7	NULL	NULL	0	NULL	P & lt ; 0.01 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Feed conversion ( P & lt ; 0.01 ) and egg production ( P & lt ; 0.01 ) improved most when both zinc and pyridoxine were supplemented to the diet .
	manualset3
224563	3	420968	7	NULL	NULL	0	NULL	egg production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Feed conversion ( P & lt ; 0.01 ) and egg production ( P & lt ; 0.01 ) improved most when both zinc and pyridoxine were supplemented to the diet .
	manualset3
224564	4	420968	7	NULL	NULL	0	NULL	P & lt ; 0.01	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Feed conversion ( P & lt ; 0.01 ) and egg production ( P & lt ; 0.01 ) improved most when both zinc and pyridoxine were supplemented to the diet .
	manualset3
224565	5	420968	7	NULL	NULL	0	NULL	zinc	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Feed conversion ( P & lt ; 0.01 ) and egg production ( P & lt ; 0.01 ) improved most when both zinc and pyridoxine were supplemented to the diet .
	manualset3
224566	6	420968	7	NULL	NULL	0	NULL	pyridoxine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Feed conversion ( P & lt ; 0.01 ) and egg production ( P & lt ; 0.01 ) improved most when both zinc and pyridoxine were supplemented to the diet .
	manualset3
224567	7	420968	7	NULL	NULL	0	NULL	diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Feed conversion ( P & lt ; 0.01 ) and egg production ( P & lt ; 0.01 ) improved most when both zinc and pyridoxine were supplemented to the diet .
	manualset3
224568	1	420969	7	NULL	NULL	0	NULL	Immunohistochemical evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical and proteomic evaluation of nuclear ubiquitous casein and cyclin-dependent kinases substrate in invasive ductal carcinoma of the breast .
	manualset3
224569	2	420969	7	NULL	NULL	0	NULL	proteomic evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical and proteomic evaluation of nuclear ubiquitous casein and cyclin-dependent kinases substrate in invasive ductal carcinoma of the breast .
	manualset3
224570	3	420969	7	NULL	NULL	0	NULL	nuclear ubiquitous casein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical and proteomic evaluation of nuclear ubiquitous casein and cyclin-dependent kinases substrate in invasive ductal carcinoma of the breast .
	manualset3
224571	4	420969	7	NULL	NULL	0	NULL	cyclin-dependent kinases substrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical and proteomic evaluation of nuclear ubiquitous casein and cyclin-dependent kinases substrate in invasive ductal carcinoma of the breast .
	manualset3
224572	5	420969	7	NULL	NULL	0	NULL	invasive ductal carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical and proteomic evaluation of nuclear ubiquitous casein and cyclin-dependent kinases substrate in invasive ductal carcinoma of the breast .
	manualset3
224573	6	420969	7	NULL	NULL	0	NULL	breast	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunohistochemical and proteomic evaluation of nuclear ubiquitous casein and cyclin-dependent kinases substrate in invasive ductal carcinoma of the breast .
	manualset3
224574	1	420970	7	NULL	NULL	0	NULL	fluorescent light	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The fluorescent light is emitted through the metal film only at an SPCE angle .
	manualset3
224575	2	420970	7	NULL	NULL	0	NULL	metal film	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The fluorescent light is emitted through the metal film only at an SPCE angle .
	manualset3
224576	3	420970	7	NULL	NULL	0	NULL	SPCE angle	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The fluorescent light is emitted through the metal film only at an SPCE angle .
	manualset3
224577	1	420971	7	NULL	NULL	0	NULL	baffled microtiter plate	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The baffled microtiter plate : increased oxygen transfer and improved online monitoring in small scale fermentations .
	manualset3
224578	2	420971	7	NULL	NULL	0	NULL	oxygen transfer 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The baffled microtiter plate : increased oxygen transfer and improved online monitoring in small scale fermentations .
	manualset3
224579	3	420971	7	NULL	NULL	0	NULL	online monitoring	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The baffled microtiter plate : increased oxygen transfer and improved online monitoring in small scale fermentations .
	manualset3
224580	4	420971	7	NULL	NULL	0	NULL	small scale fermentations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The baffled microtiter plate : increased oxygen transfer and improved online monitoring in small scale fermentations .
	manualset3
224581	1	420972	7	NULL	NULL	0	NULL	brief report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	( A brief report on the prevention of urological complications iin paraplegics ) .
	manualset3
224582	2	420972	7	NULL	NULL	0	NULL	prevention 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( A brief report on the prevention of urological complications iin paraplegics ) .
	manualset3
224583	3	420972	7	NULL	NULL	0	NULL	 urological complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( A brief report on the prevention of urological complications iin paraplegics ) .
	manualset3
224584	4	420972	7	NULL	NULL	0	NULL	paraplegics	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( A brief report on the prevention of urological complications iin paraplegics ) .
	manualset3
224585	1	420973	7	NULL	NULL	0	NULL	multidrug-resistant ( MDR ) Salmonella Heidelberg isolates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the multidrug-resistant ( MDR ) Salmonella Heidelberg isolates , Class 1 integrons with variable sizes of 1.2 to 1.5 kb were detected in six isolates ( three each ) from humans and swine .
	manualset3
224586	2	420973	7	NULL	NULL	0	NULL	Class 1 integrons	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the multidrug-resistant ( MDR ) Salmonella Heidelberg isolates , Class 1 integrons with variable sizes of 1.2 to 1.5 kb were detected in six isolates ( three each ) from humans and swine .
	manualset3
224587	3	420973	7	NULL	NULL	0	NULL	variable sizes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the multidrug-resistant ( MDR ) Salmonella Heidelberg isolates , Class 1 integrons with variable sizes of 1.2 to 1.5 kb were detected in six isolates ( three each ) from humans and swine .
	manualset3
224588	4	420973	7	NULL	NULL	0	NULL	1.2 kb	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the multidrug-resistant ( MDR ) Salmonella Heidelberg isolates , Class 1 integrons with variable sizes of 1.2 to 1.5 kb were detected in six isolates ( three each ) from humans and swine .
	manualset3
224589	5	420973	7	NULL	NULL	0	NULL	1.5 kb	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the multidrug-resistant ( MDR ) Salmonella Heidelberg isolates , Class 1 integrons with variable sizes of 1.2 to 1.5 kb were detected in six isolates ( three each ) from humans and swine .
	manualset3
224590	6	420973	7	NULL	NULL	0	NULL	 six isolates 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the multidrug-resistant ( MDR ) Salmonella Heidelberg isolates , Class 1 integrons with variable sizes of 1.2 to 1.5 kb were detected in six isolates ( three each ) from humans and swine .
	manualset3
224591	7	420973	7	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the multidrug-resistant ( MDR ) Salmonella Heidelberg isolates , Class 1 integrons with variable sizes of 1.2 to 1.5 kb were detected in six isolates ( three each ) from humans and swine .
	manualset3
224592	8	420973	7	NULL	NULL	0	NULL	humans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the multidrug-resistant ( MDR ) Salmonella Heidelberg isolates , Class 1 integrons with variable sizes of 1.2 to 1.5 kb were detected in six isolates ( three each ) from humans and swine .
	manualset3
224593	9	420973	7	NULL	NULL	0	NULL	swine	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the multidrug-resistant ( MDR ) Salmonella Heidelberg isolates , Class 1 integrons with variable sizes of 1.2 to 1.5 kb were detected in six isolates ( three each ) from humans and swine .
	manualset3
224594	1	420974	7	NULL	NULL	0	NULL	histology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The histology of the tumor grafts was intermediate between fibrosarcoma and lymphosarcoma .
	manualset3
224595	2	420974	7	NULL	NULL	0	NULL	tumor grafts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The histology of the tumor grafts was intermediate between fibrosarcoma and lymphosarcoma .
	manualset3
224596	3	420974	7	NULL	NULL	0	NULL	fibrosarcoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The histology of the tumor grafts was intermediate between fibrosarcoma and lymphosarcoma .
	manualset3
224597	4	420974	7	NULL	NULL	0	NULL	lymphosarcoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The histology of the tumor grafts was intermediate between fibrosarcoma and lymphosarcoma .
	manualset3
224598	1	420975	7	NULL	NULL	0	NULL	six	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For six of these complexes , the DeltaGdegrees ( H - ) values calculated using heterolytic activation of hydrogen are compared with those based on thermodynamic cycles using pK ( a ) measurements and electrochemical half-wave potentials .
	manualset3
224599	2	420975	7	NULL	NULL	0	NULL	complexes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For six of these complexes , the DeltaGdegrees ( H - ) values calculated using heterolytic activation of hydrogen are compared with those based on thermodynamic cycles using pK ( a ) measurements and electrochemical half-wave potentials .
	manualset3
224600	3	420975	7	NULL	NULL	0	NULL	 DeltaGdegrees ( H - ) values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For six of these complexes , the DeltaGdegrees ( H - ) values calculated using heterolytic activation of hydrogen are compared with those based on thermodynamic cycles using pK ( a ) measurements and electrochemical half-wave potentials .
	manualset3
224601	4	420975	7	NULL	NULL	NULL	NULL	heterolytic activation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For six of these complexes , the DeltaGdegrees ( H - ) values calculated using heterolytic activation of hydrogen are compared with those based on thermodynamic cycles using pK ( a ) measurements and electrochemical half-wave potentials .
	manualset3
224602	5	420975	7	NULL	NULL	0	NULL	hydrogen	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For six of these complexes , the DeltaGdegrees ( H - ) values calculated using heterolytic activation of hydrogen are compared with those based on thermodynamic cycles using pK ( a ) measurements and electrochemical half-wave potentials .
	manualset3
224603	6	420975	7	NULL	NULL	0	NULL	 thermodynamic cycles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For six of these complexes , the DeltaGdegrees ( H - ) values calculated using heterolytic activation of hydrogen are compared with those based on thermodynamic cycles using pK ( a ) measurements and electrochemical half-wave potentials .
	manualset3
224604	7	420975	7	NULL	NULL	0	NULL	pK ( a ) measurements	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For six of these complexes , the DeltaGdegrees ( H - ) values calculated using heterolytic activation of hydrogen are compared with those based on thermodynamic cycles using pK ( a ) measurements and electrochemical half-wave potentials .
	manualset3
224605	8	420975	7	NULL	NULL	0	NULL	electrochemical half-wave potentials 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	For six of these complexes , the DeltaGdegrees ( H - ) values calculated using heterolytic activation of hydrogen are compared with those based on thermodynamic cycles using pK ( a ) measurements and electrochemical half-wave potentials .
	manualset3
224606	1	420976	7	NULL	NULL	0	NULL	 majority	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the majority of survivors suffer long-term side-effects due to severe management modalities .
	manualset3
224607	2	420976	7	NULL	NULL	0	NULL	survivors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the majority of survivors suffer long-term side-effects due to severe management modalities .
	manualset3
224608	3	420976	7	NULL	NULL	0	NULL	long-term side-effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the majority of survivors suffer long-term side-effects due to severe management modalities .
	manualset3
224609	4	420976	7	NULL	NULL	0	NULL	 severe management modalities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the majority of survivors suffer long-term side-effects due to severe management modalities .
	manualset3
224610	1	420977	7	NULL	NULL	0	NULL	heterogeneity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Despite this heterogeneity all are found to contain a homologous region ( s ) defined by DNA/DNA hybridization .
	manualset3
224611	2	420977	7	NULL	NULL	0	NULL	homologous region ( s )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Despite this heterogeneity all are found to contain a homologous region ( s ) defined by DNA/DNA hybridization .
	manualset3
224612	3	420977	7	NULL	NULL	NULL	NULL	DNA/DNA hybridization	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this heterogeneity all are found to contain a homologous region ( s ) defined by DNA/DNA hybridization .
	manualset3
224613	1	420978	7	NULL	NULL	0	NULL	Baseline characteristics	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Baseline characteristics included myopia ( 10 eyes ; range , 5.00 to 15.00 diopters ) and perforating trauma ( one eye ) .
	manualset3
224614	2	420978	7	NULL	NULL	0	NULL	myopia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Baseline characteristics included myopia ( 10 eyes ; range , 5.00 to 15.00 diopters ) and perforating trauma ( one eye ) .
	manualset3
224615	3	420978	7	NULL	NULL	0	NULL	10 eyes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Baseline characteristics included myopia ( 10 eyes ; range , 5.00 to 15.00 diopters ) and perforating trauma ( one eye ) .
	manualset3
224616	4	420978	7	NULL	NULL	0	NULL	 range 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Baseline characteristics included myopia ( 10 eyes ; range , 5.00 to 15.00 diopters ) and perforating trauma ( one eye ) .
	manualset3
224617	5	420978	7	NULL	NULL	0	NULL	5.00 diopters	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Baseline characteristics included myopia ( 10 eyes ; range , 5.00 to 15.00 diopters ) and perforating trauma ( one eye ) .
	manualset3
224618	6	420978	7	NULL	NULL	0	NULL	15.00 diopters	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Baseline characteristics included myopia ( 10 eyes ; range , 5.00 to 15.00 diopters ) and perforating trauma ( one eye ) .
	manualset3
224619	7	420978	7	NULL	NULL	0	NULL	trauma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Baseline characteristics included myopia ( 10 eyes ; range , 5.00 to 15.00 diopters ) and perforating trauma ( one eye ) .
	manualset3
224620	8	420978	7	NULL	NULL	0	NULL	one eye	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Baseline characteristics included myopia ( 10 eyes ; range , 5.00 to 15.00 diopters ) and perforating trauma ( one eye ) .
	manualset3
224621	1	420979	7	NULL	NULL	0	NULL	pollutants	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the pollutants tested are metals ( mercury and copper ) and various organic compounds ( chlorophenols , toluene , polycyclic aromatic hydrocarbons , tetradifon and pyridine ) ; organisms include mussels , oysters , earthworms , water fleas and zebrafish .
	manualset3
224622	2	420979	7	NULL	NULL	0	NULL	metals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the pollutants tested are metals ( mercury and copper ) and various organic compounds ( chlorophenols , toluene , polycyclic aromatic hydrocarbons , tetradifon and pyridine ) ; organisms include mussels , oysters , earthworms , water fleas and zebrafish .
	manualset3
224623	3	420979	7	NULL	NULL	0	NULL	mercury	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the pollutants tested are metals ( mercury and copper ) and various organic compounds ( chlorophenols , toluene , polycyclic aromatic hydrocarbons , tetradifon and pyridine ) ; organisms include mussels , oysters , earthworms , water fleas and zebrafish .
	manualset3
224624	4	420979	7	NULL	NULL	0	NULL	copper 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the pollutants tested are metals ( mercury and copper ) and various organic compounds ( chlorophenols , toluene , polycyclic aromatic hydrocarbons , tetradifon and pyridine ) ; organisms include mussels , oysters , earthworms , water fleas and zebrafish .
	manualset3
224625	5	420979	7	NULL	NULL	0	NULL	organic compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the pollutants tested are metals ( mercury and copper ) and various organic compounds ( chlorophenols , toluene , polycyclic aromatic hydrocarbons , tetradifon and pyridine ) ; organisms include mussels , oysters , earthworms , water fleas and zebrafish .
	manualset3
224626	6	420979	7	NULL	NULL	0	NULL	chlorophenols	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the pollutants tested are metals ( mercury and copper ) and various organic compounds ( chlorophenols , toluene , polycyclic aromatic hydrocarbons , tetradifon and pyridine ) ; organisms include mussels , oysters , earthworms , water fleas and zebrafish .
	manualset3
224627	7	420979	7	NULL	NULL	0	NULL	toluene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the pollutants tested are metals ( mercury and copper ) and various organic compounds ( chlorophenols , toluene , polycyclic aromatic hydrocarbons , tetradifon and pyridine ) ; organisms include mussels , oysters , earthworms , water fleas and zebrafish .
	manualset3
224628	8	420979	7	NULL	NULL	0	NULL	polycyclic aromatic hydrocarbons	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the pollutants tested are metals ( mercury and copper ) and various organic compounds ( chlorophenols , toluene , polycyclic aromatic hydrocarbons , tetradifon and pyridine ) ; organisms include mussels , oysters , earthworms , water fleas and zebrafish .
	manualset3
224629	9	420979	7	NULL	NULL	0	NULL	tetradifon	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the pollutants tested are metals ( mercury and copper ) and various organic compounds ( chlorophenols , toluene , polycyclic aromatic hydrocarbons , tetradifon and pyridine ) ; organisms include mussels , oysters , earthworms , water fleas and zebrafish .
	manualset3
224630	10	420979	7	NULL	NULL	0	NULL	pyridine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the pollutants tested are metals ( mercury and copper ) and various organic compounds ( chlorophenols , toluene , polycyclic aromatic hydrocarbons , tetradifon and pyridine ) ; organisms include mussels , oysters , earthworms , water fleas and zebrafish .
	manualset3
224631	11	420979	7	NULL	NULL	0	NULL	organisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the pollutants tested are metals ( mercury and copper ) and various organic compounds ( chlorophenols , toluene , polycyclic aromatic hydrocarbons , tetradifon and pyridine ) ; organisms include mussels , oysters , earthworms , water fleas and zebrafish .
	manualset3
224632	12	420979	7	NULL	NULL	0	NULL	mussels	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the pollutants tested are metals ( mercury and copper ) and various organic compounds ( chlorophenols , toluene , polycyclic aromatic hydrocarbons , tetradifon and pyridine ) ; organisms include mussels , oysters , earthworms , water fleas and zebrafish .
	manualset3
224633	13	420979	7	NULL	NULL	0	NULL	oysters	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the pollutants tested are metals ( mercury and copper ) and various organic compounds ( chlorophenols , toluene , polycyclic aromatic hydrocarbons , tetradifon and pyridine ) ; organisms include mussels , oysters , earthworms , water fleas and zebrafish .
	manualset3
224634	14	420979	7	NULL	NULL	0	NULL	earthworms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the pollutants tested are metals ( mercury and copper ) and various organic compounds ( chlorophenols , toluene , polycyclic aromatic hydrocarbons , tetradifon and pyridine ) ; organisms include mussels , oysters , earthworms , water fleas and zebrafish .
	manualset3
224635	15	420979	7	NULL	NULL	0	NULL	water fleas	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the pollutants tested are metals ( mercury and copper ) and various organic compounds ( chlorophenols , toluene , polycyclic aromatic hydrocarbons , tetradifon and pyridine ) ; organisms include mussels , oysters , earthworms , water fleas and zebrafish .
	manualset3
224636	16	420979	7	NULL	NULL	0	NULL	zebrafish 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the pollutants tested are metals ( mercury and copper ) and various organic compounds ( chlorophenols , toluene , polycyclic aromatic hydrocarbons , tetradifon and pyridine ) ; organisms include mussels , oysters , earthworms , water fleas and zebrafish .
	manualset3
224637	1	420980	7	NULL	NULL	0	NULL	Lactogenic hormones	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Lactogenic hormones induced the appearance of larger droplets that occurred in intracytoplasmic lumens and lipid synthesis rates were initially increased .
	manualset3
224638	2	420980	7	NULL	NULL	0	NULL	appearance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Lactogenic hormones induced the appearance of larger droplets that occurred in intracytoplasmic lumens and lipid synthesis rates were initially increased .
	manualset3
224639	3	420980	7	NULL	NULL	0	NULL	larger droplets	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lactogenic hormones induced the appearance of larger droplets that occurred in intracytoplasmic lumens and lipid synthesis rates were initially increased .
	manualset3
224640	4	420980	7	NULL	NULL	0	NULL	intracytoplasmic lumens	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Lactogenic hormones induced the appearance of larger droplets that occurred in intracytoplasmic lumens and lipid synthesis rates were initially increased .
	manualset3
224641	5	420980	7	NULL	NULL	0	NULL	lipid synthesis rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Lactogenic hormones induced the appearance of larger droplets that occurred in intracytoplasmic lumens and lipid synthesis rates were initially increased .
	manualset3
224642	1	420981	7	NULL	NULL	0	NULL	Donor age	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Donor age greater than 50 years does not influence midterm results of heart transplantation .
	manualset3
224643	2	420981	7	NULL	NULL	0	NULL	50 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Donor age greater than 50 years does not influence midterm results of heart transplantation .
	manualset3
224644	3	420981	7	NULL	NULL	0	NULL	midterm results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Donor age greater than 50 years does not influence midterm results of heart transplantation .
	manualset3
224645	4	420981	7	NULL	NULL	0	NULL	heart transplantation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Donor age greater than 50 years does not influence midterm results of heart transplantation .
	manualset3
224646	1	420982	7	NULL	NULL	0	NULL	central composite design	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A central composite design was used to optimize the enzyme-assisted extraction of lycopene from the peel fraction of tomato processing waste .
	manualset3
224647	2	420982	7	NULL	NULL	0	NULL	enzyme-assisted extraction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A central composite design was used to optimize the enzyme-assisted extraction of lycopene from the peel fraction of tomato processing waste .
	manualset3
224648	3	420982	7	NULL	NULL	0	NULL	 lycopene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A central composite design was used to optimize the enzyme-assisted extraction of lycopene from the peel fraction of tomato processing waste .
	manualset3
224649	4	420982	7	NULL	NULL	0	NULL	peel fraction	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A central composite design was used to optimize the enzyme-assisted extraction of lycopene from the peel fraction of tomato processing waste .
	manualset3
224650	5	420982	7	NULL	NULL	0	NULL	tomato processing waste	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A central composite design was used to optimize the enzyme-assisted extraction of lycopene from the peel fraction of tomato processing waste .
	manualset3
224651	1	420983	7	NULL	NULL	0	NULL	 effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This effect was observed at concentrations of 0.05-5 microM , ranges where this compound is effective at inhibiting HMG-CoA reductase .
	manualset3
224652	2	420983	7	NULL	NULL	0	NULL	concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This effect was observed at concentrations of 0.05-5 microM , ranges where this compound is effective at inhibiting HMG-CoA reductase .
	manualset3
224653	3	420983	7	NULL	NULL	0	NULL	0.05-5 microM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This effect was observed at concentrations of 0.05-5 microM , ranges where this compound is effective at inhibiting HMG-CoA reductase .
	manualset3
224654	4	420983	7	NULL	NULL	0	NULL	 ranges	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This effect was observed at concentrations of 0.05-5 microM , ranges where this compound is effective at inhibiting HMG-CoA reductase .
	manualset3
224655	5	420983	7	NULL	NULL	0	NULL	compound 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This effect was observed at concentrations of 0.05-5 microM , ranges where this compound is effective at inhibiting HMG-CoA reductase .
	manualset3
224656	6	420983	7	NULL	NULL	0	NULL	HMG-CoA reductase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This effect was observed at concentrations of 0.05-5 microM , ranges where this compound is effective at inhibiting HMG-CoA reductase .
	manualset3
224657	1	420984	7	NULL	NULL	0	NULL	Marked goblet cell hyperplasia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked goblet cell hyperplasia with mucus accumulation in the airways of patients who died of severe acute asthma attack .
	manualset3
224658	2	420984	7	NULL	NULL	0	NULL	mucus accumulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked goblet cell hyperplasia with mucus accumulation in the airways of patients who died of severe acute asthma attack .
	manualset3
224659	3	420984	7	NULL	NULL	0	NULL	airways	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked goblet cell hyperplasia with mucus accumulation in the airways of patients who died of severe acute asthma attack .
	manualset3
224660	4	420984	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked goblet cell hyperplasia with mucus accumulation in the airways of patients who died of severe acute asthma attack .
	manualset3
224661	5	420984	7	NULL	NULL	0	NULL	severe acute asthma attack	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Marked goblet cell hyperplasia with mucus accumulation in the airways of patients who died of severe acute asthma attack .
	manualset3
224662	1	420985	7	NULL	NULL	0	NULL	New World monkeys 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	New World monkeys : Cebidae : ( 1 ) Saimiri sciureus ( squirrel monkey ) ; ( 2 ) Lagothrix lagothricha ( Humboldt 's woolly monkey ) .
	manualset3
224663	2	420985	7	NULL	NULL	0	NULL	Cebidae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	New World monkeys : Cebidae : ( 1 ) Saimiri sciureus ( squirrel monkey ) ; ( 2 ) Lagothrix lagothricha ( Humboldt 's woolly monkey ) .
	manualset3
224664	3	420985	7	NULL	NULL	0	NULL	 Saimiri sciureus ( squirrel monkey )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	New World monkeys : Cebidae : ( 1 ) Saimiri sciureus ( squirrel monkey ) ; ( 2 ) Lagothrix lagothricha ( Humboldt 's woolly monkey ) .
	manualset3
224665	4	420985	7	NULL	NULL	0	NULL	Lagothrix lagothricha ( Humboldt 's woolly monkey )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	New World monkeys : Cebidae : ( 1 ) Saimiri sciureus ( squirrel monkey ) ; ( 2 ) Lagothrix lagothricha ( Humboldt 's woolly monkey ) .
	manualset3
224666	1	420986	7	NULL	NULL	0	NULL	Progress	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Progress in cloning , expression and purification of 5-enolpyruvylshikimate-3-phosphate synthase from pathogens causing meningitis .
	manualset3
224667	2	420986	7	NULL	NULL	0	NULL	cloning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Progress in cloning , expression and purification of 5-enolpyruvylshikimate-3-phosphate synthase from pathogens causing meningitis .
	manualset3
224668	3	420986	7	NULL	NULL	0	NULL	expression 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Progress in cloning , expression and purification of 5-enolpyruvylshikimate-3-phosphate synthase from pathogens causing meningitis .
	manualset3
224669	4	420986	7	NULL	NULL	0	NULL	purification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Progress in cloning , expression and purification of 5-enolpyruvylshikimate-3-phosphate synthase from pathogens causing meningitis .
	manualset3
224670	5	420986	7	NULL	NULL	0	NULL	5-enolpyruvylshikimate-3-phosphate synthase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Progress in cloning , expression and purification of 5-enolpyruvylshikimate-3-phosphate synthase from pathogens causing meningitis .
	manualset3
224671	6	420986	7	NULL	NULL	0	NULL	 pathogens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Progress in cloning , expression and purification of 5-enolpyruvylshikimate-3-phosphate synthase from pathogens causing meningitis .
	manualset3
224672	7	420986	7	NULL	NULL	0	NULL	meningitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Progress in cloning , expression and purification of 5-enolpyruvylshikimate-3-phosphate synthase from pathogens causing meningitis .
	manualset3
224673	1	420987	7	NULL	NULL	0	NULL	present studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present studies compared the effects of the non-competitive NMDA antagonist dextrorphan ( Dex ) and the kappa-selective opioid antagonist nor-binaltorphimine ( nor-BNI ) on the acute motor deficits and chronic neuropathological alterations caused by intrathecally administered dynorphin A - ( 1-17 ) ( Dyn A ) .
	manualset3
224674	2	420987	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present studies compared the effects of the non-competitive NMDA antagonist dextrorphan ( Dex ) and the kappa-selective opioid antagonist nor-binaltorphimine ( nor-BNI ) on the acute motor deficits and chronic neuropathological alterations caused by intrathecally administered dynorphin A - ( 1-17 ) ( Dyn A ) .
	manualset3
224675	3	420987	7	NULL	NULL	0	NULL	non-competitive NMDA antagonist dextrorphan ( Dex )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The present studies compared the effects of the non-competitive NMDA antagonist dextrorphan ( Dex ) and the kappa-selective opioid antagonist nor-binaltorphimine ( nor-BNI ) on the acute motor deficits and chronic neuropathological alterations caused by intrathecally administered dynorphin A - ( 1-17 ) ( Dyn A ) .
	manualset3
224676	4	420987	7	NULL	NULL	0	NULL	kappa-selective opioid antagonist nor-binaltorphimine ( nor-BNI )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The present studies compared the effects of the non-competitive NMDA antagonist dextrorphan ( Dex ) and the kappa-selective opioid antagonist nor-binaltorphimine ( nor-BNI ) on the acute motor deficits and chronic neuropathological alterations caused by intrathecally administered dynorphin A - ( 1-17 ) ( Dyn A ) .
	manualset3
224677	5	420987	7	NULL	NULL	0	NULL	acute motor deficits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present studies compared the effects of the non-competitive NMDA antagonist dextrorphan ( Dex ) and the kappa-selective opioid antagonist nor-binaltorphimine ( nor-BNI ) on the acute motor deficits and chronic neuropathological alterations caused by intrathecally administered dynorphin A - ( 1-17 ) ( Dyn A ) .
	manualset3
224678	6	420987	7	NULL	NULL	0	NULL	chronic neuropathological alterations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present studies compared the effects of the non-competitive NMDA antagonist dextrorphan ( Dex ) and the kappa-selective opioid antagonist nor-binaltorphimine ( nor-BNI ) on the acute motor deficits and chronic neuropathological alterations caused by intrathecally administered dynorphin A - ( 1-17 ) ( Dyn A ) .
	manualset3
224679	7	420987	7	NULL	NULL	0	NULL	dynorphin A - ( 1-17 ) ( Dyn A )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The present studies compared the effects of the non-competitive NMDA antagonist dextrorphan ( Dex ) and the kappa-selective opioid antagonist nor-binaltorphimine ( nor-BNI ) on the acute motor deficits and chronic neuropathological alterations caused by intrathecally administered dynorphin A - ( 1-17 ) ( Dyn A ) .
	manualset3
224680	1	420988	7	NULL	NULL	0	NULL	MLOs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the remaining MLOs used in this study , Vinca virescence and elm yellows MLOs may be very distantly related , if at all , to BB MLO .
	manualset3
224681	2	420988	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the remaining MLOs used in this study , Vinca virescence and elm yellows MLOs may be very distantly related , if at all , to BB MLO .
	manualset3
224682	3	420988	7	NULL	NULL	0	NULL	Vinca virescence	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the remaining MLOs used in this study , Vinca virescence and elm yellows MLOs may be very distantly related , if at all , to BB MLO .
	manualset3
224683	4	420988	7	NULL	NULL	0	NULL	elm yellows MLOs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the remaining MLOs used in this study , Vinca virescence and elm yellows MLOs may be very distantly related , if at all , to BB MLO .
	manualset3
224684	5	420988	7	NULL	NULL	0	NULL	BB MLO	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the remaining MLOs used in this study , Vinca virescence and elm yellows MLOs may be very distantly related , if at all , to BB MLO .
	manualset3
224685	1	420989	7	NULL	NULL	0	NULL	glial fibrillary acidic protein ( GFAP ) staining	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous glial fibrillary acidic protein ( GFAP ) staining of mirror sections was performed .
	manualset3
224686	2	420989	7	NULL	NULL	0	NULL	mirror sections 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneous glial fibrillary acidic protein ( GFAP ) staining of mirror sections was performed .
	manualset3
224687	1	420990	7	NULL	NULL	0	NULL	 lack 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This was because of the lack of a reliable and efficient mammalian cell-based in vitro DNA replication system .
	manualset3
224688	2	420990	7	NULL	NULL	0	NULL	 mammalian cell-based in vitro DNA replication system	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	This was because of the lack of a reliable and efficient mammalian cell-based in vitro DNA replication system .
	manualset3
224689	1	420991	7	NULL	NULL	0	NULL	alpha response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The alpha response consists of a slowing of rate , the beta response of an acceleration of rate and hyperpolarization of RAF .
	manualset3
224690	2	420991	7	NULL	NULL	0	NULL	slowing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The alpha response consists of a slowing of rate , the beta response of an acceleration of rate and hyperpolarization of RAF .
	manualset3
224691	3	420991	7	NULL	NULL	0	NULL	rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The alpha response consists of a slowing of rate , the beta response of an acceleration of rate and hyperpolarization of RAF .
	manualset3
224692	4	420991	7	NULL	NULL	0	NULL	beta response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The alpha response consists of a slowing of rate , the beta response of an acceleration of rate and hyperpolarization of RAF .
	manualset3
224693	5	420991	7	NULL	NULL	0	NULL	acceleration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The alpha response consists of a slowing of rate , the beta response of an acceleration of rate and hyperpolarization of RAF .
	manualset3
224694	6	420991	7	NULL	NULL	0	NULL	rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The alpha response consists of a slowing of rate , the beta response of an acceleration of rate and hyperpolarization of RAF .
	manualset3
224695	7	420991	7	NULL	NULL	0	NULL	hyperpolarization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The alpha response consists of a slowing of rate , the beta response of an acceleration of rate and hyperpolarization of RAF .
	manualset3
224696	8	420991	7	NULL	NULL	0	NULL	RAF	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The alpha response consists of a slowing of rate , the beta response of an acceleration of rate and hyperpolarization of RAF .
	manualset3
224697	1	420992	7	NULL	NULL	0	NULL	Posterior fossa arachnoid cysts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Posterior fossa arachnoid cysts : two case reports .
	manualset3
224698	2	420992	7	NULL	NULL	0	NULL	two case reports	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Posterior fossa arachnoid cysts : two case reports .
	manualset3
224699	1	420993	7	NULL	NULL	0	NULL	 finding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This finding is different from the growth inhibition of these cells induced by elevated calcium levels ( 1.5 mM ) which was tightly coupled to terminal differentiation .
	manualset3
224700	2	420993	7	NULL	NULL	0	NULL	growth inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This finding is different from the growth inhibition of these cells induced by elevated calcium levels ( 1.5 mM ) which was tightly coupled to terminal differentiation .
	manualset3
224701	3	420993	7	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	This finding is different from the growth inhibition of these cells induced by elevated calcium levels ( 1.5 mM ) which was tightly coupled to terminal differentiation .
	manualset3
224702	4	420993	7	NULL	NULL	0	NULL	elevated calcium levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This finding is different from the growth inhibition of these cells induced by elevated calcium levels ( 1.5 mM ) which was tightly coupled to terminal differentiation .
	manualset3
224703	5	420993	7	NULL	NULL	0	NULL	1.5 mM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This finding is different from the growth inhibition of these cells induced by elevated calcium levels ( 1.5 mM ) which was tightly coupled to terminal differentiation .
	manualset3
224704	6	420993	7	NULL	NULL	0	NULL	terminal differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This finding is different from the growth inhibition of these cells induced by elevated calcium levels ( 1.5 mM ) which was tightly coupled to terminal differentiation .
	manualset3
224705	1	420994	7	NULL	NULL	0	NULL	abnormal differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The abnormal differentiation of NSCs would lead to CNS disorders .
	manualset3
224706	2	420994	7	NULL	NULL	0	NULL	NSCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The abnormal differentiation of NSCs would lead to CNS disorders .
	manualset3
224707	3	420994	7	NULL	NULL	0	NULL	CNS disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The abnormal differentiation of NSCs would lead to CNS disorders .
	manualset3
224708	1	420995	7	NULL	NULL	0	NULL	repertoire 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the repertoire of motor functions , although hand movement and speech production tasks have been investigated widely by functional neuroimaging , paradigms combining both movements have been studied less so .
	manualset3
224709	2	420995	7	NULL	NULL	0	NULL	motor functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the repertoire of motor functions , although hand movement and speech production tasks have been investigated widely by functional neuroimaging , paradigms combining both movements have been studied less so .
	manualset3
224710	3	420995	7	NULL	NULL	0	NULL	hand movement	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the repertoire of motor functions , although hand movement and speech production tasks have been investigated widely by functional neuroimaging , paradigms combining both movements have been studied less so .
	manualset3
224711	4	420995	7	NULL	NULL	NULL	NULL	speech production tasks	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Among the repertoire of motor functions , although hand movement and speech production tasks have been investigated widely by functional neuroimaging , paradigms combining both movements have been studied less so .
	manualset3
224712	5	420995	7	NULL	NULL	0	NULL	functional neuroimaging 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the repertoire of motor functions , although hand movement and speech production tasks have been investigated widely by functional neuroimaging , paradigms combining both movements have been studied less so .
	manualset3
224713	6	420995	7	NULL	NULL	0	NULL	movements	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the repertoire of motor functions , although hand movement and speech production tasks have been investigated widely by functional neuroimaging , paradigms combining both movements have been studied less so .
	manualset3
226673	7	420995	7	NULL	NULL	0	NULL	 paradigms	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the repertoire of motor functions , although hand movement and speech production tasks have been investigated widely by functional neuroimaging , paradigms combining both movements have been studied less so .
	manualset3
224714	1	420996	7	NULL	NULL	0	NULL	 measurement 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A simultaneous measurement of blood velocity was performed to allow determination of the blood flow .
	manualset3
224715	2	420996	7	NULL	NULL	0	NULL	blood velocity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A simultaneous measurement of blood velocity was performed to allow determination of the blood flow .
	manualset3
224716	3	420996	7	NULL	NULL	0	NULL	determination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A simultaneous measurement of blood velocity was performed to allow determination of the blood flow .
	manualset3
224717	4	420996	7	NULL	NULL	0	NULL	blood flow	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A simultaneous measurement of blood velocity was performed to allow determination of the blood flow .
	manualset3
224718	1	420997	7	NULL	NULL	0	NULL	immunohistochemistry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	As shown by immunohistochemistry , the CXCR4 immunopositive neurons were distributed in all layers and areas of hippocampal formation .
	manualset3
224719	2	420997	7	NULL	NULL	0	NULL	CXCR4 immunopositive neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	As shown by immunohistochemistry , the CXCR4 immunopositive neurons were distributed in all layers and areas of hippocampal formation .
	manualset3
224720	3	420997	7	NULL	NULL	0	NULL	all layers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	As shown by immunohistochemistry , the CXCR4 immunopositive neurons were distributed in all layers and areas of hippocampal formation .
	manualset3
224721	4	420997	7	NULL	NULL	0	NULL	areas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	As shown by immunohistochemistry , the CXCR4 immunopositive neurons were distributed in all layers and areas of hippocampal formation .
	manualset3
224722	5	420997	7	NULL	NULL	0	NULL	hippocampal formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As shown by immunohistochemistry , the CXCR4 immunopositive neurons were distributed in all layers and areas of hippocampal formation .
	manualset3
224944	1	420998	7	NULL	NULL	0	NULL	proinflammatory shift	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , a proinflammatory shift in the profile of vascular cytokine expression may contribute to the aging-induced phenotypic changes in coronary arteries , promoting the development of ischemic heart disease in the elderly .
	manualset3
224945	2	420998	7	NULL	NULL	0	NULL	profile	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , a proinflammatory shift in the profile of vascular cytokine expression may contribute to the aging-induced phenotypic changes in coronary arteries , promoting the development of ischemic heart disease in the elderly .
	manualset3
224946	3	420998	7	NULL	NULL	0	NULL	vascular cytokine expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , a proinflammatory shift in the profile of vascular cytokine expression may contribute to the aging-induced phenotypic changes in coronary arteries , promoting the development of ischemic heart disease in the elderly .
	manualset3
224947	4	420998	7	NULL	NULL	0	NULL	aging-induced phenotypic changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , a proinflammatory shift in the profile of vascular cytokine expression may contribute to the aging-induced phenotypic changes in coronary arteries , promoting the development of ischemic heart disease in the elderly .
	manualset3
224948	5	420998	7	NULL	NULL	0	NULL	coronary arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , a proinflammatory shift in the profile of vascular cytokine expression may contribute to the aging-induced phenotypic changes in coronary arteries , promoting the development of ischemic heart disease in the elderly .
	manualset3
224949	6	420998	7	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , a proinflammatory shift in the profile of vascular cytokine expression may contribute to the aging-induced phenotypic changes in coronary arteries , promoting the development of ischemic heart disease in the elderly .
	manualset3
224950	7	420998	7	NULL	NULL	0	NULL	ischemic heart disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , a proinflammatory shift in the profile of vascular cytokine expression may contribute to the aging-induced phenotypic changes in coronary arteries , promoting the development of ischemic heart disease in the elderly .
	manualset3
224951	8	420998	7	NULL	NULL	0	NULL	elderly 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , a proinflammatory shift in the profile of vascular cytokine expression may contribute to the aging-induced phenotypic changes in coronary arteries , promoting the development of ischemic heart disease in the elderly .
	manualset3
224952	1	420999	7	NULL	NULL	0	NULL	members	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Some members of DZ twin pairs born to mixed-race couples inherit very different physical features from their parents .
	manualset3
224953	2	420999	7	NULL	NULL	0	NULL	DZ twin pairs	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Some members of DZ twin pairs born to mixed-race couples inherit very different physical features from their parents .
	manualset3
224954	3	420999	7	NULL	NULL	0	NULL	mixed-race couples	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Some members of DZ twin pairs born to mixed-race couples inherit very different physical features from their parents .
	manualset3
224955	4	420999	7	NULL	NULL	0	NULL	 different physical features	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some members of DZ twin pairs born to mixed-race couples inherit very different physical features from their parents .
	manualset3
224956	5	420999	7	NULL	NULL	0	NULL	parents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Some members of DZ twin pairs born to mixed-race couples inherit very different physical features from their parents .
	manualset3
224957	1	421000	7	NULL	NULL	0	NULL	Mean S	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean S ( Iclamp ) was 44.41 x 10 ( -4 ) x l ( -2 ) min ( -1 ) x mU ( -1 ) ( range 22.0-77 .92 ) .
	manualset3
224958	2	421000	7	NULL	NULL	NULL	NULL	44.41 x 10 ( -4 ) x l ( -2 ) min ( -1 ) x mU ( -1 )	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mean S ( Iclamp ) was 44.41 x 10 ( -4 ) x l ( -2 ) min ( -1 ) x mU ( -1 ) ( range 22.0-77 .92 ) .
	manualset3
224959	3	421000	7	NULL	NULL	0	NULL	range 22.0-77 .92	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean S ( Iclamp ) was 44.41 x 10 ( -4 ) x l ( -2 ) min ( -1 ) x mU ( -1 ) ( range 22.0-77 .92 ) .
	manualset3
224960	4	421000	7	NULL	NULL	0	NULL	Iclamp	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mean S ( Iclamp ) was 44.41 x 10 ( -4 ) x l ( -2 ) min ( -1 ) x mU ( -1 ) ( range 22.0-77 .92 ) .
	manualset3
225029	1	421001	7	NULL	NULL	0	NULL	Clinical indications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical indications of chromatic qualitative perimetry ) .
	manualset3
225030	2	421001	7	NULL	NULL	0	NULL	chromatic qualitative perimetry 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical indications of chromatic qualitative perimetry ) .
	manualset3
225031	1	421002	7	NULL	NULL	0	NULL	 adenosine stress cardiovascular magnetic resonance	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Because adenosine stress cardiovascular magnetic resonance is currently the most widely used clinically , it is the primary focus of this article .
	manualset3
225032	2	421002	7	NULL	NULL	0	NULL	primary focus	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Because adenosine stress cardiovascular magnetic resonance is currently the most widely used clinically , it is the primary focus of this article .
	manualset3
225033	3	421002	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Because adenosine stress cardiovascular magnetic resonance is currently the most widely used clinically , it is the primary focus of this article .
	manualset3
225034	1	421003	7	NULL	NULL	0	NULL	actions 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfortunatly the actions of systematic detection of new cases are not sufficient and the sanitary education is almost non existent .
	manualset3
225035	2	421003	7	NULL	NULL	0	NULL	systematic detection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfortunatly the actions of systematic detection of new cases are not sufficient and the sanitary education is almost non existent .
	manualset3
225036	3	421003	7	NULL	NULL	0	NULL	new cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfortunatly the actions of systematic detection of new cases are not sufficient and the sanitary education is almost non existent .
	manualset3
225037	4	421003	7	NULL	NULL	0	NULL	 sanitary education	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Unfortunatly the actions of systematic detection of new cases are not sufficient and the sanitary education is almost non existent .
	manualset3
225038	1	421004	7	NULL	NULL	0	NULL	Special attention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention is devoted to the automatic relevance determination ( ARD ) to reduce input variable numbers , which avoid the use of principal component analysis .
	manualset3
225039	2	421004	7	NULL	NULL	0	NULL	automatic relevance determination ( ARD )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention is devoted to the automatic relevance determination ( ARD ) to reduce input variable numbers , which avoid the use of principal component analysis .
	manualset3
225040	3	421004	7	NULL	NULL	0	NULL	 input variable numbers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention is devoted to the automatic relevance determination ( ARD ) to reduce input variable numbers , which avoid the use of principal component analysis .
	manualset3
225041	4	421004	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention is devoted to the automatic relevance determination ( ARD ) to reduce input variable numbers , which avoid the use of principal component analysis .
	manualset3
225042	5	421004	7	NULL	NULL	0	NULL	principal component analysis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Special attention is devoted to the automatic relevance determination ( ARD ) to reduce input variable numbers , which avoid the use of principal component analysis .
	manualset3
225043	1	421005	7	NULL	NULL	0	NULL	set 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the set of six closely linked late genes , marked differences were observed in both the levels of transcription and the kinetic patterns of expression , providing direct evidence for the existence of differentially regulated gene subsets within the late gene class .
	manualset3
225044	2	421005	7	NULL	NULL	0	NULL	six closely linked late genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the set of six closely linked late genes , marked differences were observed in both the levels of transcription and the kinetic patterns of expression , providing direct evidence for the existence of differentially regulated gene subsets within the late gene class .
	manualset3
225045	3	421005	7	NULL	NULL	0	NULL	marked differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the set of six closely linked late genes , marked differences were observed in both the levels of transcription and the kinetic patterns of expression , providing direct evidence for the existence of differentially regulated gene subsets within the late gene class .
	manualset3
225046	4	421005	7	NULL	NULL	0	NULL	levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the set of six closely linked late genes , marked differences were observed in both the levels of transcription and the kinetic patterns of expression , providing direct evidence for the existence of differentially regulated gene subsets within the late gene class .
	manualset3
225047	5	421005	7	NULL	NULL	0	NULL	transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the set of six closely linked late genes , marked differences were observed in both the levels of transcription and the kinetic patterns of expression , providing direct evidence for the existence of differentially regulated gene subsets within the late gene class .
	manualset3
225048	6	421005	7	NULL	NULL	0	NULL	kinetic patterns 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the set of six closely linked late genes , marked differences were observed in both the levels of transcription and the kinetic patterns of expression , providing direct evidence for the existence of differentially regulated gene subsets within the late gene class .
	manualset3
225049	7	421005	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the set of six closely linked late genes , marked differences were observed in both the levels of transcription and the kinetic patterns of expression , providing direct evidence for the existence of differentially regulated gene subsets within the late gene class .
	manualset3
225050	8	421005	7	NULL	NULL	0	NULL	direct evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the set of six closely linked late genes , marked differences were observed in both the levels of transcription and the kinetic patterns of expression , providing direct evidence for the existence of differentially regulated gene subsets within the late gene class .
	manualset3
225051	9	421005	7	NULL	NULL	0	NULL	existence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the set of six closely linked late genes , marked differences were observed in both the levels of transcription and the kinetic patterns of expression , providing direct evidence for the existence of differentially regulated gene subsets within the late gene class .
	manualset3
225052	10	421005	7	NULL	NULL	0	NULL	differentially regulated gene subsets	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the set of six closely linked late genes , marked differences were observed in both the levels of transcription and the kinetic patterns of expression , providing direct evidence for the existence of differentially regulated gene subsets within the late gene class .
	manualset3
225053	11	421005	7	NULL	NULL	0	NULL	late gene class	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the set of six closely linked late genes , marked differences were observed in both the levels of transcription and the kinetic patterns of expression , providing direct evidence for the existence of differentially regulated gene subsets within the late gene class .
	manualset3
225054	1	421006	7	NULL	NULL	0	NULL	DFT study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	DFT study of nitroxide radicals : explicit modeling of solvent effects on the structural and electronic characteristics of 4-amino-2 , 2 , 6 , 6 - tetramethyl-piperidine-N-oxyl .
	manualset3
225055	2	421006	7	NULL	NULL	0	NULL	nitroxide radicals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	DFT study of nitroxide radicals : explicit modeling of solvent effects on the structural and electronic characteristics of 4-amino-2 , 2 , 6 , 6 - tetramethyl-piperidine-N-oxyl .
	manualset3
225056	3	421006	7	NULL	NULL	0	NULL	explicit modeling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	DFT study of nitroxide radicals : explicit modeling of solvent effects on the structural and electronic characteristics of 4-amino-2 , 2 , 6 , 6 - tetramethyl-piperidine-N-oxyl .
	manualset3
225057	4	421006	7	NULL	NULL	0	NULL	solvent effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	DFT study of nitroxide radicals : explicit modeling of solvent effects on the structural and electronic characteristics of 4-amino-2 , 2 , 6 , 6 - tetramethyl-piperidine-N-oxyl .
	manualset3
225058	5	421006	7	NULL	NULL	0	NULL	 4-amino-2 , 2 , 6 , 6 - tetramethyl-piperidine-N-oxyl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	DFT study of nitroxide radicals : explicit modeling of solvent effects on the structural and electronic characteristics of 4-amino-2 , 2 , 6 , 6 - tetramethyl-piperidine-N-oxyl .
	manualset3
226674	6	421006	7	NULL	NULL	NULL	NULL	structural characteristics	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DFT study of nitroxide radicals : explicit modeling of solvent effects on the structural and electronic characteristics of 4-amino-2 , 2 , 6 , 6 - tetramethyl-piperidine-N-oxyl .
	manualset3
226675	7	421006	7	NULL	NULL	0	NULL	electronic characteristics	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	DFT study of nitroxide radicals : explicit modeling of solvent effects on the structural and electronic characteristics of 4-amino-2 , 2 , 6 , 6 - tetramethyl-piperidine-N-oxyl .
	manualset3
225059	1	421007	7	NULL	NULL	0	NULL	single intravenous injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A single intravenous injection of KRN5500 ( antibiotic spicamycin ) produces long-term decreases in multiple sensory hypersensitivities in neuropathic pain .
	manualset3
225060	2	421007	7	NULL	NULL	0	NULL	KRN5500 ( antibiotic spicamycin )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A single intravenous injection of KRN5500 ( antibiotic spicamycin ) produces long-term decreases in multiple sensory hypersensitivities in neuropathic pain .
	manualset3
225061	3	421007	7	NULL	NULL	0	NULL	long-term decreases	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A single intravenous injection of KRN5500 ( antibiotic spicamycin ) produces long-term decreases in multiple sensory hypersensitivities in neuropathic pain .
	manualset3
225062	4	421007	7	NULL	NULL	0	NULL	multiple sensory hypersensitivities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A single intravenous injection of KRN5500 ( antibiotic spicamycin ) produces long-term decreases in multiple sensory hypersensitivities in neuropathic pain .
	manualset3
225063	5	421007	7	NULL	NULL	0	NULL	neuropathic pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A single intravenous injection of KRN5500 ( antibiotic spicamycin ) produces long-term decreases in multiple sensory hypersensitivities in neuropathic pain .
	manualset3
225064	1	421008	7	NULL	NULL	0	NULL	Fifty-one patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Fifty-one patients were correctly assessed as having a clear duct and unsuspected residual calculi were demonstrated by choledochoscopy in 13 patients .
	manualset3
225065	2	421008	7	NULL	NULL	0	NULL	clear duct	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Fifty-one patients were correctly assessed as having a clear duct and unsuspected residual calculi were demonstrated by choledochoscopy in 13 patients .
	manualset3
225066	3	421008	7	NULL	NULL	0	NULL	unsuspected residual calculi	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Fifty-one patients were correctly assessed as having a clear duct and unsuspected residual calculi were demonstrated by choledochoscopy in 13 patients .
	manualset3
225067	4	421008	7	NULL	NULL	0	NULL	choledochoscopy	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Fifty-one patients were correctly assessed as having a clear duct and unsuspected residual calculi were demonstrated by choledochoscopy in 13 patients .
	manualset3
225068	5	421008	7	NULL	NULL	0	NULL	13 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Fifty-one patients were correctly assessed as having a clear duct and unsuspected residual calculi were demonstrated by choledochoscopy in 13 patients .
	manualset3
225069	1	421009	7	NULL	NULL	0	NULL	Subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were instructed to rotate their heads in a sinusoidal-like manner and to focus their attention on producing a smooth head rotation .
	manualset3
225070	2	421009	7	NULL	NULL	0	NULL	heads	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were instructed to rotate their heads in a sinusoidal-like manner and to focus their attention on producing a smooth head rotation .
	manualset3
225071	3	421009	7	NULL	NULL	0	NULL	 sinusoidal-like manner	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were instructed to rotate their heads in a sinusoidal-like manner and to focus their attention on producing a smooth head rotation .
	manualset3
225072	4	421009	7	NULL	NULL	0	NULL	attention	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were instructed to rotate their heads in a sinusoidal-like manner and to focus their attention on producing a smooth head rotation .
	manualset3
225073	5	421009	7	NULL	NULL	0	NULL	smooth head rotation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subjects were instructed to rotate their heads in a sinusoidal-like manner and to focus their attention on producing a smooth head rotation .
	manualset3
225074	1	421010	7	NULL	NULL	0	NULL	 precarious condition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	They appeared to be more unbalanced and in more precarious condition than subjects treated in specialized care centers but they were not representative of the patients maintained by buprenorphine .
	manualset3
225075	2	421010	7	NULL	NULL	0	NULL	subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	They appeared to be more unbalanced and in more precarious condition than subjects treated in specialized care centers but they were not representative of the patients maintained by buprenorphine .
	manualset3
225076	3	421010	7	NULL	NULL	0	NULL	specialized care centers	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	They appeared to be more unbalanced and in more precarious condition than subjects treated in specialized care centers but they were not representative of the patients maintained by buprenorphine .
	manualset3
225077	4	421010	7	NULL	NULL	0	NULL	 representative	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	They appeared to be more unbalanced and in more precarious condition than subjects treated in specialized care centers but they were not representative of the patients maintained by buprenorphine .
	manualset3
225078	5	421010	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	They appeared to be more unbalanced and in more precarious condition than subjects treated in specialized care centers but they were not representative of the patients maintained by buprenorphine .
	manualset3
225079	6	421010	7	NULL	NULL	0	NULL	buprenorphine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	They appeared to be more unbalanced and in more precarious condition than subjects treated in specialized care centers but they were not representative of the patients maintained by buprenorphine .
	manualset3
225080	1	421011	7	NULL	NULL	0	NULL	Evaluating	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluating the NMDA-glutamate receptor as a site of action for toluene , in vivo .
	manualset3
225081	2	421011	7	NULL	NULL	0	NULL	NMDA-glutamate receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluating the NMDA-glutamate receptor as a site of action for toluene , in vivo .
	manualset3
225082	3	421011	7	NULL	NULL	0	NULL	site of action	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluating the NMDA-glutamate receptor as a site of action for toluene , in vivo .
	manualset3
225083	4	421011	7	NULL	NULL	0	NULL	toluene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluating the NMDA-glutamate receptor as a site of action for toluene , in vivo .
	manualset3
225084	1	421012	7	NULL	NULL	0	NULL	seven risk factors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the seven risk factors analyzed , altitude was the main predictor of birth weight ( except for gestational age ) .
	manualset3
225085	2	421012	7	NULL	NULL	0	NULL	altitude	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the seven risk factors analyzed , altitude was the main predictor of birth weight ( except for gestational age ) .
	manualset3
225086	3	421012	7	NULL	NULL	0	NULL	main predictor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the seven risk factors analyzed , altitude was the main predictor of birth weight ( except for gestational age ) .
	manualset3
225087	4	421012	7	NULL	NULL	0	NULL	birth weight	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the seven risk factors analyzed , altitude was the main predictor of birth weight ( except for gestational age ) .
	manualset3
225088	5	421012	7	NULL	NULL	0	NULL	gestational age	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the seven risk factors analyzed , altitude was the main predictor of birth weight ( except for gestational age ) .
	manualset3
225089	1	421013	7	NULL	NULL	0	NULL	introduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The introduction of human brain functions such as perception and cognition into the computer has been made possible by the use of Artificial Neural Network ( ANN ) .
	manualset3
225090	2	421013	7	NULL	NULL	0	NULL	human brain functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The introduction of human brain functions such as perception and cognition into the computer has been made possible by the use of Artificial Neural Network ( ANN ) .
	manualset3
225091	3	421013	7	NULL	NULL	0	NULL	perception	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The introduction of human brain functions such as perception and cognition into the computer has been made possible by the use of Artificial Neural Network ( ANN ) .
	manualset3
225092	4	421013	7	NULL	NULL	0	NULL	cognition	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The introduction of human brain functions such as perception and cognition into the computer has been made possible by the use of Artificial Neural Network ( ANN ) .
	manualset3
225093	5	421013	7	NULL	NULL	0	NULL	computer	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The introduction of human brain functions such as perception and cognition into the computer has been made possible by the use of Artificial Neural Network ( ANN ) .
	manualset3
225094	6	421013	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The introduction of human brain functions such as perception and cognition into the computer has been made possible by the use of Artificial Neural Network ( ANN ) .
	manualset3
225095	7	421013	7	NULL	NULL	0	NULL	Artificial Neural Network ( ANN ) 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The introduction of human brain functions such as perception and cognition into the computer has been made possible by the use of Artificial Neural Network ( ANN ) .
	manualset3
225096	1	421014	7	NULL	NULL	0	NULL	Selective inactivation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective inactivation of one RC shows that the responses of the contralateral RC are not due to electrotonic coupling between the two cells , but to synaptic actions impinging upon the membrane of both RCs .
	manualset3
225097	2	421014	7	NULL	NULL	0	NULL	one 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective inactivation of one RC shows that the responses of the contralateral RC are not due to electrotonic coupling between the two cells , but to synaptic actions impinging upon the membrane of both RCs .
	manualset3
225098	3	421014	7	NULL	NULL	0	NULL	RC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective inactivation of one RC shows that the responses of the contralateral RC are not due to electrotonic coupling between the two cells , but to synaptic actions impinging upon the membrane of both RCs .
	manualset3
225099	4	421014	7	NULL	NULL	0	NULL	 responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective inactivation of one RC shows that the responses of the contralateral RC are not due to electrotonic coupling between the two cells , but to synaptic actions impinging upon the membrane of both RCs .
	manualset3
225100	5	421014	7	NULL	NULL	0	NULL	contralateral RC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective inactivation of one RC shows that the responses of the contralateral RC are not due to electrotonic coupling between the two cells , but to synaptic actions impinging upon the membrane of both RCs .
	manualset3
225101	6	421014	7	NULL	NULL	0	NULL	electrotonic coupling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective inactivation of one RC shows that the responses of the contralateral RC are not due to electrotonic coupling between the two cells , but to synaptic actions impinging upon the membrane of both RCs .
	manualset3
225102	7	421014	7	NULL	NULL	0	NULL	two cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective inactivation of one RC shows that the responses of the contralateral RC are not due to electrotonic coupling between the two cells , but to synaptic actions impinging upon the membrane of both RCs .
	manualset3
225103	8	421014	7	NULL	NULL	0	NULL	synaptic actions 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective inactivation of one RC shows that the responses of the contralateral RC are not due to electrotonic coupling between the two cells , but to synaptic actions impinging upon the membrane of both RCs .
	manualset3
225104	9	421014	7	NULL	NULL	0	NULL	membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective inactivation of one RC shows that the responses of the contralateral RC are not due to electrotonic coupling between the two cells , but to synaptic actions impinging upon the membrane of both RCs .
	manualset3
225105	10	421014	7	NULL	NULL	0	NULL	RCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective inactivation of one RC shows that the responses of the contralateral RC are not due to electrotonic coupling between the two cells , but to synaptic actions impinging upon the membrane of both RCs .
	manualset3
225106	1	421015	7	NULL	NULL	0	NULL	Artemisinin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Artemisinin isolated from the aerial parts of Artemisia annua L. , is a promising and potent antimalarial drug , which meets the dual challenge posed by drug-resistant parasites and rapid progression of malarial illness .
	manualset3
225107	2	421015	7	NULL	NULL	0	NULL	aerial parts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Artemisinin isolated from the aerial parts of Artemisia annua L. , is a promising and potent antimalarial drug , which meets the dual challenge posed by drug-resistant parasites and rapid progression of malarial illness .
	manualset3
225108	3	421015	7	NULL	NULL	0	NULL	Artemisia annua L. ,	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Artemisinin isolated from the aerial parts of Artemisia annua L. , is a promising and potent antimalarial drug , which meets the dual challenge posed by drug-resistant parasites and rapid progression of malarial illness .
	manualset3
225109	4	421015	7	NULL	NULL	0	NULL	antimalarial drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Artemisinin isolated from the aerial parts of Artemisia annua L. , is a promising and potent antimalarial drug , which meets the dual challenge posed by drug-resistant parasites and rapid progression of malarial illness .
	manualset3
225110	5	421015	7	NULL	NULL	0	NULL	dual challenge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Artemisinin isolated from the aerial parts of Artemisia annua L. , is a promising and potent antimalarial drug , which meets the dual challenge posed by drug-resistant parasites and rapid progression of malarial illness .
	manualset3
225111	6	421015	7	NULL	NULL	0	NULL	drug-resistant parasites	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Artemisinin isolated from the aerial parts of Artemisia annua L. , is a promising and potent antimalarial drug , which meets the dual challenge posed by drug-resistant parasites and rapid progression of malarial illness .
	manualset3
225112	7	421015	7	NULL	NULL	0	NULL	rapid progression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Artemisinin isolated from the aerial parts of Artemisia annua L. , is a promising and potent antimalarial drug , which meets the dual challenge posed by drug-resistant parasites and rapid progression of malarial illness .
	manualset3
225113	8	421015	7	NULL	NULL	0	NULL	malarial illness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Artemisinin isolated from the aerial parts of Artemisia annua L. , is a promising and potent antimalarial drug , which meets the dual challenge posed by drug-resistant parasites and rapid progression of malarial illness .
	manualset3
225114	1	421016	7	NULL	NULL	0	NULL	 understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , based on recent advances in our understanding of the neurobiology of relapse and published preclinical data , we highlight the most promising areas for future anti-relapse medication development .
	manualset3
225115	2	421016	7	NULL	NULL	0	NULL	neurobiology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , based on recent advances in our understanding of the neurobiology of relapse and published preclinical data , we highlight the most promising areas for future anti-relapse medication development .
	manualset3
225116	3	421016	7	NULL	NULL	0	NULL	relapse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , based on recent advances in our understanding of the neurobiology of relapse and published preclinical data , we highlight the most promising areas for future anti-relapse medication development .
	manualset3
225117	4	421016	7	NULL	NULL	0	NULL	 published preclinical data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , based on recent advances in our understanding of the neurobiology of relapse and published preclinical data , we highlight the most promising areas for future anti-relapse medication development .
	manualset3
225118	5	421016	7	NULL	NULL	0	NULL	promising areas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , based on recent advances in our understanding of the neurobiology of relapse and published preclinical data , we highlight the most promising areas for future anti-relapse medication development .
	manualset3
225119	6	421016	7	NULL	NULL	0	NULL	anti-relapse medication development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , based on recent advances in our understanding of the neurobiology of relapse and published preclinical data , we highlight the most promising areas for future anti-relapse medication development .
	manualset3
225120	7	421016	7	NULL	NULL	0	NULL	 recent advances	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Finally , based on recent advances in our understanding of the neurobiology of relapse and published preclinical data , we highlight the most promising areas for future anti-relapse medication development .
	manualset3
225121	1	421017	7	NULL	NULL	0	NULL	Grating acuity	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Grating acuity was tested binocularly at 0-1 month and monocularly at 4 , 9 , 12 , 18 , 24 , 30 , 36 and 48 months corrected age , using Teller acuity cards .
	manualset3
225122	2	421017	7	NULL	NULL	0	NULL	 0-1 month	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Grating acuity was tested binocularly at 0-1 month and monocularly at 4 , 9 , 12 , 18 , 24 , 30 , 36 and 48 months corrected age , using Teller acuity cards .
	manualset3
225123	3	421017	7	NULL	NULL	0	NULL	 4 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Grating acuity was tested binocularly at 0-1 month and monocularly at 4 , 9 , 12 , 18 , 24 , 30 , 36 and 48 months corrected age , using Teller acuity cards .
	manualset3
225124	4	421017	7	NULL	NULL	0	NULL	9 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Grating acuity was tested binocularly at 0-1 month and monocularly at 4 , 9 , 12 , 18 , 24 , 30 , 36 and 48 months corrected age , using Teller acuity cards .
	manualset3
225125	5	421017	7	NULL	NULL	0	NULL	12 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Grating acuity was tested binocularly at 0-1 month and monocularly at 4 , 9 , 12 , 18 , 24 , 30 , 36 and 48 months corrected age , using Teller acuity cards .
	manualset3
225126	6	421017	7	NULL	NULL	0	NULL	18 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Grating acuity was tested binocularly at 0-1 month and monocularly at 4 , 9 , 12 , 18 , 24 , 30 , 36 and 48 months corrected age , using Teller acuity cards .
	manualset3
225127	7	421017	7	NULL	NULL	0	NULL	 24 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Grating acuity was tested binocularly at 0-1 month and monocularly at 4 , 9 , 12 , 18 , 24 , 30 , 36 and 48 months corrected age , using Teller acuity cards .
	manualset3
225128	8	421017	7	NULL	NULL	0	NULL	30 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Grating acuity was tested binocularly at 0-1 month and monocularly at 4 , 9 , 12 , 18 , 24 , 30 , 36 and 48 months corrected age , using Teller acuity cards .
	manualset3
225129	9	421017	7	NULL	NULL	0	NULL	 36 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Grating acuity was tested binocularly at 0-1 month and monocularly at 4 , 9 , 12 , 18 , 24 , 30 , 36 and 48 months corrected age , using Teller acuity cards .
	manualset3
225130	10	421017	7	NULL	NULL	0	NULL	48 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Grating acuity was tested binocularly at 0-1 month and monocularly at 4 , 9 , 12 , 18 , 24 , 30 , 36 and 48 months corrected age , using Teller acuity cards .
	manualset3
225131	11	421017	7	NULL	NULL	0	NULL	corrected age 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Grating acuity was tested binocularly at 0-1 month and monocularly at 4 , 9 , 12 , 18 , 24 , 30 , 36 and 48 months corrected age , using Teller acuity cards .
	manualset3
225132	12	421017	7	NULL	NULL	0	NULL	Teller acuity cards	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Grating acuity was tested binocularly at 0-1 month and monocularly at 4 , 9 , 12 , 18 , 24 , 30 , 36 and 48 months corrected age , using Teller acuity cards .
	manualset3
225133	1	421018	7	NULL	NULL	0	NULL	 evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is abundant evidence that these multifunctional signaling adapters also mediate inhibitory activity , downmodulating signaling from Toll-like receptors and other heterologous receptors .
	manualset3
225134	2	421018	7	NULL	NULL	0	NULL	multifunctional signaling adapters	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	There is abundant evidence that these multifunctional signaling adapters also mediate inhibitory activity , downmodulating signaling from Toll-like receptors and other heterologous receptors .
	manualset3
225135	3	421018	7	NULL	NULL	0	NULL	inhibitory activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There is abundant evidence that these multifunctional signaling adapters also mediate inhibitory activity , downmodulating signaling from Toll-like receptors and other heterologous receptors .
	manualset3
225136	4	421018	7	NULL	NULL	0	NULL	downmodulating signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There is abundant evidence that these multifunctional signaling adapters also mediate inhibitory activity , downmodulating signaling from Toll-like receptors and other heterologous receptors .
	manualset3
225137	5	421018	7	NULL	NULL	0	NULL	Toll-like receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There is abundant evidence that these multifunctional signaling adapters also mediate inhibitory activity , downmodulating signaling from Toll-like receptors and other heterologous receptors .
	manualset3
225138	6	421018	7	NULL	NULL	0	NULL	heterologous receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There is abundant evidence that these multifunctional signaling adapters also mediate inhibitory activity , downmodulating signaling from Toll-like receptors and other heterologous receptors .
	manualset3
225139	1	421019	7	NULL	NULL	0	NULL	Review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Review : developmental origins of neural tumors : old idea , new approaches .
	manualset3
225140	2	421019	7	NULL	NULL	0	NULL	developmental origins 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Review : developmental origins of neural tumors : old idea , new approaches .
	manualset3
225141	3	421019	7	NULL	NULL	0	NULL	neural tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Review : developmental origins of neural tumors : old idea , new approaches .
	manualset3
225142	4	421019	7	NULL	NULL	0	NULL	old idea	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Review : developmental origins of neural tumors : old idea , new approaches .
	manualset3
225143	5	421019	7	NULL	NULL	0	NULL	new approaches	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Review : developmental origins of neural tumors : old idea , new approaches .
	manualset3
225144	1	421020	7	NULL	NULL	0	NULL	facultative bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the facultative bacteria capable of growth on mesquite wood which were isolated from the asceptically dissected hind-gut of the termite Reticulitermes hesperus were two strains of Bacillus cereus , one strain each of Arthrobacter , Alcaligenes and Serratia , and a very small Gram-negative fermentative rod .
	manualset3
225145	2	421020	7	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the facultative bacteria capable of growth on mesquite wood which were isolated from the asceptically dissected hind-gut of the termite Reticulitermes hesperus were two strains of Bacillus cereus , one strain each of Arthrobacter , Alcaligenes and Serratia , and a very small Gram-negative fermentative rod .
	manualset3
225146	3	421020	7	NULL	NULL	0	NULL	mesquite wood	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the facultative bacteria capable of growth on mesquite wood which were isolated from the asceptically dissected hind-gut of the termite Reticulitermes hesperus were two strains of Bacillus cereus , one strain each of Arthrobacter , Alcaligenes and Serratia , and a very small Gram-negative fermentative rod .
	manualset3
225147	4	421020	7	NULL	NULL	0	NULL	dissected hind-gut 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the facultative bacteria capable of growth on mesquite wood which were isolated from the asceptically dissected hind-gut of the termite Reticulitermes hesperus were two strains of Bacillus cereus , one strain each of Arthrobacter , Alcaligenes and Serratia , and a very small Gram-negative fermentative rod .
	manualset3
225148	5	421020	7	NULL	NULL	0	NULL	termite Reticulitermes hesperus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the facultative bacteria capable of growth on mesquite wood which were isolated from the asceptically dissected hind-gut of the termite Reticulitermes hesperus were two strains of Bacillus cereus , one strain each of Arthrobacter , Alcaligenes and Serratia , and a very small Gram-negative fermentative rod .
	manualset3
225149	6	421020	7	NULL	NULL	0	NULL	two strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the facultative bacteria capable of growth on mesquite wood which were isolated from the asceptically dissected hind-gut of the termite Reticulitermes hesperus were two strains of Bacillus cereus , one strain each of Arthrobacter , Alcaligenes and Serratia , and a very small Gram-negative fermentative rod .
	manualset3
225150	7	421020	7	NULL	NULL	0	NULL	Bacillus cereus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the facultative bacteria capable of growth on mesquite wood which were isolated from the asceptically dissected hind-gut of the termite Reticulitermes hesperus were two strains of Bacillus cereus , one strain each of Arthrobacter , Alcaligenes and Serratia , and a very small Gram-negative fermentative rod .
	manualset3
225151	8	421020	7	NULL	NULL	0	NULL	 one strain 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the facultative bacteria capable of growth on mesquite wood which were isolated from the asceptically dissected hind-gut of the termite Reticulitermes hesperus were two strains of Bacillus cereus , one strain each of Arthrobacter , Alcaligenes and Serratia , and a very small Gram-negative fermentative rod .
	manualset3
225152	9	421020	7	NULL	NULL	0	NULL	Arthrobacter	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the facultative bacteria capable of growth on mesquite wood which were isolated from the asceptically dissected hind-gut of the termite Reticulitermes hesperus were two strains of Bacillus cereus , one strain each of Arthrobacter , Alcaligenes and Serratia , and a very small Gram-negative fermentative rod .
	manualset3
225153	10	421020	7	NULL	NULL	0	NULL	Alcaligenes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the facultative bacteria capable of growth on mesquite wood which were isolated from the asceptically dissected hind-gut of the termite Reticulitermes hesperus were two strains of Bacillus cereus , one strain each of Arthrobacter , Alcaligenes and Serratia , and a very small Gram-negative fermentative rod .
	manualset3
225154	11	421020	7	NULL	NULL	0	NULL	Serratia	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the facultative bacteria capable of growth on mesquite wood which were isolated from the asceptically dissected hind-gut of the termite Reticulitermes hesperus were two strains of Bacillus cereus , one strain each of Arthrobacter , Alcaligenes and Serratia , and a very small Gram-negative fermentative rod .
	manualset3
225155	12	421020	7	NULL	NULL	0	NULL	small Gram-negative fermentative rod	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the facultative bacteria capable of growth on mesquite wood which were isolated from the asceptically dissected hind-gut of the termite Reticulitermes hesperus were two strains of Bacillus cereus , one strain each of Arthrobacter , Alcaligenes and Serratia , and a very small Gram-negative fermentative rod .
	manualset3
225156	1	421021	7	NULL	NULL	0	NULL	strains RF/Ms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the strains RF/Ms , SWM/Ms and SWR/Ms were superior in avoidance , while C3H/HeMs , DBA/2 and DBAf/Lw were superior in discrimination .
	manualset3
225157	2	421021	7	NULL	NULL	0	NULL	SWM/Ms 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the strains RF/Ms , SWM/Ms and SWR/Ms were superior in avoidance , while C3H/HeMs , DBA/2 and DBAf/Lw were superior in discrimination .
	manualset3
225158	3	421021	7	NULL	NULL	0	NULL	SWR/Ms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the strains RF/Ms , SWM/Ms and SWR/Ms were superior in avoidance , while C3H/HeMs , DBA/2 and DBAf/Lw were superior in discrimination .
	manualset3
225159	4	421021	7	NULL	NULL	0	NULL	C3H/HeMs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the strains RF/Ms , SWM/Ms and SWR/Ms were superior in avoidance , while C3H/HeMs , DBA/2 and DBAf/Lw were superior in discrimination .
	manualset3
225160	5	421021	7	NULL	NULL	0	NULL	DBA/2	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the strains RF/Ms , SWM/Ms and SWR/Ms were superior in avoidance , while C3H/HeMs , DBA/2 and DBAf/Lw were superior in discrimination .
	manualset3
225161	6	421021	7	NULL	NULL	0	NULL	DBAf/Lw 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the strains RF/Ms , SWM/Ms and SWR/Ms were superior in avoidance , while C3H/HeMs , DBA/2 and DBAf/Lw were superior in discrimination .
	manualset3
225162	7	421021	7	NULL	NULL	0	NULL	discrimination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the strains RF/Ms , SWM/Ms and SWR/Ms were superior in avoidance , while C3H/HeMs , DBA/2 and DBAf/Lw were superior in discrimination .
	manualset3
225163	1	421022	7	NULL	NULL	0	NULL	Diffuse axonal injury ( DAI )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Diffuse axonal injury ( DAI ) , the severest form of diffuse brain injury , causes extensive damage throughout the cerebrum , diencephalon and brainstem .
	manualset3
225164	2	421022	7	NULL	NULL	0	NULL	severest form	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Diffuse axonal injury ( DAI ) , the severest form of diffuse brain injury , causes extensive damage throughout the cerebrum , diencephalon and brainstem .
	manualset3
225165	3	421022	7	NULL	NULL	0	NULL	diffuse brain injury 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Diffuse axonal injury ( DAI ) , the severest form of diffuse brain injury , causes extensive damage throughout the cerebrum , diencephalon and brainstem .
	manualset3
225166	4	421022	7	NULL	NULL	0	NULL	extensive damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Diffuse axonal injury ( DAI ) , the severest form of diffuse brain injury , causes extensive damage throughout the cerebrum , diencephalon and brainstem .
	manualset3
225167	5	421022	7	NULL	NULL	0	NULL	cerebrum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Diffuse axonal injury ( DAI ) , the severest form of diffuse brain injury , causes extensive damage throughout the cerebrum , diencephalon and brainstem .
	manualset3
225168	6	421022	7	NULL	NULL	0	NULL	diencephalon	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Diffuse axonal injury ( DAI ) , the severest form of diffuse brain injury , causes extensive damage throughout the cerebrum , diencephalon and brainstem .
	manualset3
225169	7	421022	7	NULL	NULL	0	NULL	brainstem	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Diffuse axonal injury ( DAI ) , the severest form of diffuse brain injury , causes extensive damage throughout the cerebrum , diencephalon and brainstem .
	manualset3
225170	1	421023	7	NULL	NULL	0	NULL	Calcium 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Calcium , magnesium , and colorectal cancer .
	manualset3
225171	2	421023	7	NULL	NULL	0	NULL	magnesium 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Calcium , magnesium , and colorectal cancer .
	manualset3
225172	3	421023	7	NULL	NULL	0	NULL	colorectal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Calcium , magnesium , and colorectal cancer .
	manualset3
225173	1	421024	7	NULL	NULL	0	NULL	Different CSFs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Different CSFs and ILs suppress programmed cell death ( apoptosis ) and induce cell multiplication and differentiation , and these processes of development are separately regulated .
	manualset3
225174	2	421024	7	NULL	NULL	0	NULL	ILs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Different CSFs and ILs suppress programmed cell death ( apoptosis ) and induce cell multiplication and differentiation , and these processes of development are separately regulated .
	manualset3
225175	3	421024	7	NULL	NULL	0	NULL	programmed cell death 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Different CSFs and ILs suppress programmed cell death ( apoptosis ) and induce cell multiplication and differentiation , and these processes of development are separately regulated .
	manualset3
225176	4	421024	7	NULL	NULL	0	NULL	 apoptosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Different CSFs and ILs suppress programmed cell death ( apoptosis ) and induce cell multiplication and differentiation , and these processes of development are separately regulated .
	manualset3
225177	5	421024	7	NULL	NULL	0	NULL	cell multiplication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Different CSFs and ILs suppress programmed cell death ( apoptosis ) and induce cell multiplication and differentiation , and these processes of development are separately regulated .
	manualset3
225178	6	421024	7	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Different CSFs and ILs suppress programmed cell death ( apoptosis ) and induce cell multiplication and differentiation , and these processes of development are separately regulated .
	manualset3
225179	7	421024	7	NULL	NULL	0	NULL	 processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Different CSFs and ILs suppress programmed cell death ( apoptosis ) and induce cell multiplication and differentiation , and these processes of development are separately regulated .
	manualset3
225180	8	421024	7	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Different CSFs and ILs suppress programmed cell death ( apoptosis ) and induce cell multiplication and differentiation , and these processes of development are separately regulated .
	manualset3
225181	1	421025	7	NULL	NULL	0	NULL	 precise mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , precise mechanisms of glycolytic flux and its regulation in IP remain to be elucidated .
	manualset3
225182	2	421025	7	NULL	NULL	0	NULL	glycolytic flux	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , precise mechanisms of glycolytic flux and its regulation in IP remain to be elucidated .
	manualset3
225183	3	421025	7	NULL	NULL	0	NULL	regulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , precise mechanisms of glycolytic flux and its regulation in IP remain to be elucidated .
	manualset3
225184	4	421025	7	NULL	NULL	0	NULL	IP	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , precise mechanisms of glycolytic flux and its regulation in IP remain to be elucidated .
	manualset3
225185	1	421026	7	NULL	NULL	0	NULL	differential activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was recently suggested that differential activity for memory and future thinking may be linked to differences in the phenomenal properties ( e.g. , richness of detail ) .
	manualset3
225186	2	421026	7	NULL	NULL	0	NULL	memory	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was recently suggested that differential activity for memory and future thinking may be linked to differences in the phenomenal properties ( e.g. , richness of detail ) .
	manualset3
225187	3	421026	7	NULL	NULL	0	NULL	future thinking	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was recently suggested that differential activity for memory and future thinking may be linked to differences in the phenomenal properties ( e.g. , richness of detail ) .
	manualset3
225188	4	421026	7	NULL	NULL	0	NULL	 differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	It was recently suggested that differential activity for memory and future thinking may be linked to differences in the phenomenal properties ( e.g. , richness of detail ) .
	manualset3
225189	5	421026	7	NULL	NULL	0	NULL	phenomenal properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	It was recently suggested that differential activity for memory and future thinking may be linked to differences in the phenomenal properties ( e.g. , richness of detail ) .
	manualset3
225190	6	421026	7	NULL	NULL	0	NULL	richness of detail	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	It was recently suggested that differential activity for memory and future thinking may be linked to differences in the phenomenal properties ( e.g. , richness of detail ) .
	manualset3
225191	1	421027	7	NULL	NULL	0	NULL	Matrix-assisted laser desorption ionization time-of-flight ( MALDI-TOF ) mass spectrometry ( MS )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Matrix-assisted laser desorption ionization time-of-flight ( MALDI-TOF ) mass spectrometry ( MS ) is a fast and reliable technology for the identification of microorganisms with proteomics approaches .
	manualset3
225192	2	421027	7	NULL	NULL	0	NULL	technology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Matrix-assisted laser desorption ionization time-of-flight ( MALDI-TOF ) mass spectrometry ( MS ) is a fast and reliable technology for the identification of microorganisms with proteomics approaches .
	manualset3
225193	3	421027	7	NULL	NULL	0	NULL	identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Matrix-assisted laser desorption ionization time-of-flight ( MALDI-TOF ) mass spectrometry ( MS ) is a fast and reliable technology for the identification of microorganisms with proteomics approaches .
	manualset3
225194	4	421027	7	NULL	NULL	0	NULL	microorganisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Matrix-assisted laser desorption ionization time-of-flight ( MALDI-TOF ) mass spectrometry ( MS ) is a fast and reliable technology for the identification of microorganisms with proteomics approaches .
	manualset3
225195	5	421027	7	NULL	NULL	0	NULL	proteomics approaches	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Matrix-assisted laser desorption ionization time-of-flight ( MALDI-TOF ) mass spectrometry ( MS ) is a fast and reliable technology for the identification of microorganisms with proteomics approaches .
	manualset3
225196	1	421028	7	NULL	NULL	0	NULL	 synthesized compounds 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the synthesized compounds , N ' - ( 4-phenyldiazenyl ) phenylisonicotinohydrazonyl cyanide 4f showed a significant activity toward both Gram-positive , Gram-negative bacteria and exhibit the most potent in vitro antifungal with MIC 's ( 625 g/mL ) against Aspergillus nieger .
	manualset3
225197	2	421028	7	NULL	NULL	0	NULL	N ' - ( 4-phenyldiazenyl ) phenylisonicotinohydrazonyl cyanide 4f	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the synthesized compounds , N ' - ( 4-phenyldiazenyl ) phenylisonicotinohydrazonyl cyanide 4f showed a significant activity toward both Gram-positive , Gram-negative bacteria and exhibit the most potent in vitro antifungal with MIC 's ( 625 g/mL ) against Aspergillus nieger .
	manualset3
225198	3	421028	7	NULL	NULL	0	NULL	 significant activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the synthesized compounds , N ' - ( 4-phenyldiazenyl ) phenylisonicotinohydrazonyl cyanide 4f showed a significant activity toward both Gram-positive , Gram-negative bacteria and exhibit the most potent in vitro antifungal with MIC 's ( 625 g/mL ) against Aspergillus nieger .
	manualset3
225199	4	421028	7	NULL	NULL	0	NULL	Gram-positive bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the synthesized compounds , N ' - ( 4-phenyldiazenyl ) phenylisonicotinohydrazonyl cyanide 4f showed a significant activity toward both Gram-positive , Gram-negative bacteria and exhibit the most potent in vitro antifungal with MIC 's ( 625 g/mL ) against Aspergillus nieger .
	manualset3
225200	5	421028	7	NULL	NULL	0	NULL	Gram-negative bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the synthesized compounds , N ' - ( 4-phenyldiazenyl ) phenylisonicotinohydrazonyl cyanide 4f showed a significant activity toward both Gram-positive , Gram-negative bacteria and exhibit the most potent in vitro antifungal with MIC 's ( 625 g/mL ) against Aspergillus nieger .
	manualset3
225201	6	421028	7	NULL	NULL	0	NULL	antifungal 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the synthesized compounds , N ' - ( 4-phenyldiazenyl ) phenylisonicotinohydrazonyl cyanide 4f showed a significant activity toward both Gram-positive , Gram-negative bacteria and exhibit the most potent in vitro antifungal with MIC 's ( 625 g/mL ) against Aspergillus nieger .
	manualset3
225202	7	421028	7	NULL	NULL	0	NULL	MIC 's 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the synthesized compounds , N ' - ( 4-phenyldiazenyl ) phenylisonicotinohydrazonyl cyanide 4f showed a significant activity toward both Gram-positive , Gram-negative bacteria and exhibit the most potent in vitro antifungal with MIC 's ( 625 g/mL ) against Aspergillus nieger .
	manualset3
225203	8	421028	7	NULL	NULL	0	NULL	625 g/mL 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the synthesized compounds , N ' - ( 4-phenyldiazenyl ) phenylisonicotinohydrazonyl cyanide 4f showed a significant activity toward both Gram-positive , Gram-negative bacteria and exhibit the most potent in vitro antifungal with MIC 's ( 625 g/mL ) against Aspergillus nieger .
	manualset3
225204	9	421028	7	NULL	NULL	0	NULL	Aspergillus nieger	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the synthesized compounds , N ' - ( 4-phenyldiazenyl ) phenylisonicotinohydrazonyl cyanide 4f showed a significant activity toward both Gram-positive , Gram-negative bacteria and exhibit the most potent in vitro antifungal with MIC 's ( 625 g/mL ) against Aspergillus nieger .
	manualset3
225205	1	421029	7	NULL	NULL	0	NULL	Subsequent studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent studies have shown that such in vitro generation of cytotoxic lymphocytes was dependent on the proliferative response in an MLC ( 4 ) , was genetically determined ( 5 ) , and possibly required the interaction of several subpopulations of T cells ( 6 ) .
	manualset3
225206	2	421029	7	NULL	NULL	0	NULL	 in vitro generation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent studies have shown that such in vitro generation of cytotoxic lymphocytes was dependent on the proliferative response in an MLC ( 4 ) , was genetically determined ( 5 ) , and possibly required the interaction of several subpopulations of T cells ( 6 ) .
	manualset3
225207	3	421029	7	NULL	NULL	0	NULL	cytotoxic lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent studies have shown that such in vitro generation of cytotoxic lymphocytes was dependent on the proliferative response in an MLC ( 4 ) , was genetically determined ( 5 ) , and possibly required the interaction of several subpopulations of T cells ( 6 ) .
	manualset3
225208	4	421029	7	NULL	NULL	0	NULL	proliferative response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent studies have shown that such in vitro generation of cytotoxic lymphocytes was dependent on the proliferative response in an MLC ( 4 ) , was genetically determined ( 5 ) , and possibly required the interaction of several subpopulations of T cells ( 6 ) .
	manualset3
225209	5	421029	7	NULL	NULL	NULL	NULL	MLC	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Subsequent studies have shown that such in vitro generation of cytotoxic lymphocytes was dependent on the proliferative response in an MLC ( 4 ) , was genetically determined ( 5 ) , and possibly required the interaction of several subpopulations of T cells ( 6 ) .
	manualset3
225210	6	421029	7	NULL	NULL	0	NULL	 interaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent studies have shown that such in vitro generation of cytotoxic lymphocytes was dependent on the proliferative response in an MLC ( 4 ) , was genetically determined ( 5 ) , and possibly required the interaction of several subpopulations of T cells ( 6 ) .
	manualset3
225211	7	421029	7	NULL	NULL	0	NULL	subpopulations	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent studies have shown that such in vitro generation of cytotoxic lymphocytes was dependent on the proliferative response in an MLC ( 4 ) , was genetically determined ( 5 ) , and possibly required the interaction of several subpopulations of T cells ( 6 ) .
	manualset3
225212	8	421029	7	NULL	NULL	0	NULL	T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequent studies have shown that such in vitro generation of cytotoxic lymphocytes was dependent on the proliferative response in an MLC ( 4 ) , was genetically determined ( 5 ) , and possibly required the interaction of several subpopulations of T cells ( 6 ) .
	manualset3
225213	1	421030	7	NULL	NULL	0	NULL	angiogenesis bioassays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In angiogenesis bioassays , only hESC-MSCs and fetal hMSCs were able to form capillary-like structures , which stained for smooth muscle and endothelial cell markers .
	manualset3
225214	2	421030	7	NULL	NULL	0	NULL	hESC-MSCs 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In angiogenesis bioassays , only hESC-MSCs and fetal hMSCs were able to form capillary-like structures , which stained for smooth muscle and endothelial cell markers .
	manualset3
225215	3	421030	7	NULL	NULL	0	NULL	fetal hMSCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In angiogenesis bioassays , only hESC-MSCs and fetal hMSCs were able to form capillary-like structures , which stained for smooth muscle and endothelial cell markers .
	manualset3
225216	4	421030	7	NULL	NULL	0	NULL	capillary-like structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In angiogenesis bioassays , only hESC-MSCs and fetal hMSCs were able to form capillary-like structures , which stained for smooth muscle and endothelial cell markers .
	manualset3
225217	5	421030	7	NULL	NULL	0	NULL	smooth muscle 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In angiogenesis bioassays , only hESC-MSCs and fetal hMSCs were able to form capillary-like structures , which stained for smooth muscle and endothelial cell markers .
	manualset3
225218	6	421030	7	NULL	NULL	0	NULL	endothelial cell markers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In angiogenesis bioassays , only hESC-MSCs and fetal hMSCs were able to form capillary-like structures , which stained for smooth muscle and endothelial cell markers .
	manualset3
225524	1	421031	7	NULL	NULL	0	NULL	binding potential	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding potential of hALP to hTERT promoter was confirmed by EMSA and the interacting sequence involved to -201 - to -56 - nt upstream region of the promoter .
	manualset3
225525	2	421031	7	NULL	NULL	0	NULL	 hALP promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding potential of hALP to hTERT promoter was confirmed by EMSA and the interacting sequence involved to -201 - to -56 - nt upstream region of the promoter .
	manualset3
225526	3	421031	7	NULL	NULL	0	NULL	hTERT promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding potential of hALP to hTERT promoter was confirmed by EMSA and the interacting sequence involved to -201 - to -56 - nt upstream region of the promoter .
	manualset3
225527	4	421031	7	NULL	NULL	0	NULL	EMSA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding potential of hALP to hTERT promoter was confirmed by EMSA and the interacting sequence involved to -201 - to -56 - nt upstream region of the promoter .
	manualset3
225528	5	421031	7	NULL	NULL	0	NULL	 interacting sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding potential of hALP to hTERT promoter was confirmed by EMSA and the interacting sequence involved to -201 - to -56 - nt upstream region of the promoter .
	manualset3
225529	6	421031	7	NULL	NULL	0	NULL	-201 - to -56 - nt 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding potential of hALP to hTERT promoter was confirmed by EMSA and the interacting sequence involved to -201 - to -56 - nt upstream region of the promoter .
	manualset3
225530	7	421031	7	NULL	NULL	0	NULL	upstream region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding potential of hALP to hTERT promoter was confirmed by EMSA and the interacting sequence involved to -201 - to -56 - nt upstream region of the promoter .
	manualset3
225531	8	421031	7	NULL	NULL	0	NULL	promoter 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The binding potential of hALP to hTERT promoter was confirmed by EMSA and the interacting sequence involved to -201 - to -56 - nt upstream region of the promoter .
	manualset3
225532	1	421032	7	NULL	NULL	0	NULL	 Sensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Sensitivity of Neisseria gonorrhoeae to spectinomycin ) .
	manualset3
225533	2	421032	7	NULL	NULL	0	NULL	Neisseria gonorrhoeae	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Sensitivity of Neisseria gonorrhoeae to spectinomycin ) .
	manualset3
225534	3	421032	7	NULL	NULL	0	NULL	spectinomycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Sensitivity of Neisseria gonorrhoeae to spectinomycin ) .
	manualset3
225535	1	421033	7	NULL	NULL	0	NULL	 result 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result from retinal detachment or surgical procedures , RPE comes in contact with glutamate from serum , glial release and the injured retina .
	manualset3
225536	2	421033	7	NULL	NULL	0	NULL	 retinal detachment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result from retinal detachment or surgical procedures , RPE comes in contact with glutamate from serum , glial release and the injured retina .
	manualset3
225537	3	421033	7	NULL	NULL	0	NULL	surgical procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result from retinal detachment or surgical procedures , RPE comes in contact with glutamate from serum , glial release and the injured retina .
	manualset3
225538	4	421033	7	NULL	NULL	0	NULL	RPE	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result from retinal detachment or surgical procedures , RPE comes in contact with glutamate from serum , glial release and the injured retina .
	manualset3
225539	5	421033	7	NULL	NULL	0	NULL	glutamate	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result from retinal detachment or surgical procedures , RPE comes in contact with glutamate from serum , glial release and the injured retina .
	manualset3
225540	6	421033	7	NULL	NULL	0	NULL	serum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result from retinal detachment or surgical procedures , RPE comes in contact with glutamate from serum , glial release and the injured retina .
	manualset3
225541	7	421033	7	NULL	NULL	0	NULL	glial release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result from retinal detachment or surgical procedures , RPE comes in contact with glutamate from serum , glial release and the injured retina .
	manualset3
225542	8	421033	7	NULL	NULL	0	NULL	injured retina 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result from retinal detachment or surgical procedures , RPE comes in contact with glutamate from serum , glial release and the injured retina .
	manualset3
225543	1	421034	7	NULL	NULL	0	NULL	Disturbances	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Disturbances of the fractional compounds of glycosaminoglycane in the urine of patients differs from the parameters of chromatograms of normals by a high content of fractions of heparansulfate in a relatively low level of chondroethylsulfatolike fractions .
	manualset3
225544	2	421034	7	NULL	NULL	0	NULL	fractional compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Disturbances of the fractional compounds of glycosaminoglycane in the urine of patients differs from the parameters of chromatograms of normals by a high content of fractions of heparansulfate in a relatively low level of chondroethylsulfatolike fractions .
	manualset3
225545	3	421034	7	NULL	NULL	0	NULL	glycosaminoglycane	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Disturbances of the fractional compounds of glycosaminoglycane in the urine of patients differs from the parameters of chromatograms of normals by a high content of fractions of heparansulfate in a relatively low level of chondroethylsulfatolike fractions .
	manualset3
225546	4	421034	7	NULL	NULL	0	NULL	urine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Disturbances of the fractional compounds of glycosaminoglycane in the urine of patients differs from the parameters of chromatograms of normals by a high content of fractions of heparansulfate in a relatively low level of chondroethylsulfatolike fractions .
	manualset3
225547	5	421034	7	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Disturbances of the fractional compounds of glycosaminoglycane in the urine of patients differs from the parameters of chromatograms of normals by a high content of fractions of heparansulfate in a relatively low level of chondroethylsulfatolike fractions .
	manualset3
225548	6	421034	7	NULL	NULL	0	NULL	parameters	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Disturbances of the fractional compounds of glycosaminoglycane in the urine of patients differs from the parameters of chromatograms of normals by a high content of fractions of heparansulfate in a relatively low level of chondroethylsulfatolike fractions .
	manualset3
225549	7	421034	7	NULL	NULL	0	NULL	chromatograms 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Disturbances of the fractional compounds of glycosaminoglycane in the urine of patients differs from the parameters of chromatograms of normals by a high content of fractions of heparansulfate in a relatively low level of chondroethylsulfatolike fractions .
	manualset3
225550	8	421034	7	NULL	NULL	0	NULL	normals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Disturbances of the fractional compounds of glycosaminoglycane in the urine of patients differs from the parameters of chromatograms of normals by a high content of fractions of heparansulfate in a relatively low level of chondroethylsulfatolike fractions .
	manualset3
225551	9	421034	7	NULL	NULL	0	NULL	high content 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Disturbances of the fractional compounds of glycosaminoglycane in the urine of patients differs from the parameters of chromatograms of normals by a high content of fractions of heparansulfate in a relatively low level of chondroethylsulfatolike fractions .
	manualset3
225552	10	421034	7	NULL	NULL	0	NULL	fractions 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Disturbances of the fractional compounds of glycosaminoglycane in the urine of patients differs from the parameters of chromatograms of normals by a high content of fractions of heparansulfate in a relatively low level of chondroethylsulfatolike fractions .
	manualset3
225553	11	421034	7	NULL	NULL	0	NULL	heparansulfate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Disturbances of the fractional compounds of glycosaminoglycane in the urine of patients differs from the parameters of chromatograms of normals by a high content of fractions of heparansulfate in a relatively low level of chondroethylsulfatolike fractions .
	manualset3
225554	12	421034	7	NULL	NULL	0	NULL	 low level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Disturbances of the fractional compounds of glycosaminoglycane in the urine of patients differs from the parameters of chromatograms of normals by a high content of fractions of heparansulfate in a relatively low level of chondroethylsulfatolike fractions .
	manualset3
225555	13	421034	7	NULL	NULL	NULL	NULL	chondroethylsulfatolike fractions	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Disturbances of the fractional compounds of glycosaminoglycane in the urine of patients differs from the parameters of chromatograms of normals by a high content of fractions of heparansulfate in a relatively low level of chondroethylsulfatolike fractions .
	manualset3
225556	1	421035	7	NULL	NULL	0	NULL	three size selections	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the three size selections ( sexual selection , fecundity selection and shell size ) , shell size explained the allometry , suggesting that females are more strongly subject to size selection associated with shell size availability than males .
	manualset3
225557	2	421035	7	NULL	NULL	0	NULL	sexual selection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the three size selections ( sexual selection , fecundity selection and shell size ) , shell size explained the allometry , suggesting that females are more strongly subject to size selection associated with shell size availability than males .
	manualset3
225558	3	421035	7	NULL	NULL	0	NULL	fecundity selection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the three size selections ( sexual selection , fecundity selection and shell size ) , shell size explained the allometry , suggesting that females are more strongly subject to size selection associated with shell size availability than males .
	manualset3
225559	4	421035	7	NULL	NULL	0	NULL	shell size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the three size selections ( sexual selection , fecundity selection and shell size ) , shell size explained the allometry , suggesting that females are more strongly subject to size selection associated with shell size availability than males .
	manualset3
225560	5	421035	7	NULL	NULL	0	NULL	shell size 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the three size selections ( sexual selection , fecundity selection and shell size ) , shell size explained the allometry , suggesting that females are more strongly subject to size selection associated with shell size availability than males .
	manualset3
225561	6	421035	7	NULL	NULL	0	NULL	allometry	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the three size selections ( sexual selection , fecundity selection and shell size ) , shell size explained the allometry , suggesting that females are more strongly subject to size selection associated with shell size availability than males .
	manualset3
225562	7	421035	7	NULL	NULL	0	NULL	females	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the three size selections ( sexual selection , fecundity selection and shell size ) , shell size explained the allometry , suggesting that females are more strongly subject to size selection associated with shell size availability than males .
	manualset3
225563	8	421035	7	NULL	NULL	0	NULL	 size selection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the three size selections ( sexual selection , fecundity selection and shell size ) , shell size explained the allometry , suggesting that females are more strongly subject to size selection associated with shell size availability than males .
	manualset3
225564	9	421035	7	NULL	NULL	0	NULL	shell size 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the three size selections ( sexual selection , fecundity selection and shell size ) , shell size explained the allometry , suggesting that females are more strongly subject to size selection associated with shell size availability than males .
	manualset3
225565	10	421035	7	NULL	NULL	0	NULL	males 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the three size selections ( sexual selection , fecundity selection and shell size ) , shell size explained the allometry , suggesting that females are more strongly subject to size selection associated with shell size availability than males .
	manualset3
225566	1	421036	7	NULL	NULL	NULL	NULL	aqueous phase	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The aqueous phase was able to permeate through the membrane while the microemulsion was retained by the thin selective layer .
	manualset3
225567	2	421036	7	NULL	NULL	NULL	NULL	membrane	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The aqueous phase was able to permeate through the membrane while the microemulsion was retained by the thin selective layer .
	manualset3
225568	3	421036	7	NULL	NULL	0	NULL	microemulsion	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The aqueous phase was able to permeate through the membrane while the microemulsion was retained by the thin selective layer .
	manualset3
225569	4	421036	7	NULL	NULL	0	NULL	 thin selective layer 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The aqueous phase was able to permeate through the membrane while the microemulsion was retained by the thin selective layer .
	manualset3
225570	1	421037	7	NULL	NULL	0	NULL	total histamine content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the total histamine content of the lung tissue in animals pretreated with DSCG and P. kurroa was significantly less than that in the untreated controls .
	manualset3
225571	2	421037	7	NULL	NULL	0	NULL	lung tissue 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the total histamine content of the lung tissue in animals pretreated with DSCG and P. kurroa was significantly less than that in the untreated controls .
	manualset3
225572	3	421037	7	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the total histamine content of the lung tissue in animals pretreated with DSCG and P. kurroa was significantly less than that in the untreated controls .
	manualset3
225573	4	421037	7	NULL	NULL	0	NULL	DSCG	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the total histamine content of the lung tissue in animals pretreated with DSCG and P. kurroa was significantly less than that in the untreated controls .
	manualset3
225574	5	421037	7	NULL	NULL	0	NULL	P. kurroa	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the total histamine content of the lung tissue in animals pretreated with DSCG and P. kurroa was significantly less than that in the untreated controls .
	manualset3
225575	6	421037	7	NULL	NULL	0	NULL	untreated controls	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the total histamine content of the lung tissue in animals pretreated with DSCG and P. kurroa was significantly less than that in the untreated controls .
	manualset3
225576	1	421038	7	NULL	NULL	0	NULL	Systemic antimicrobial drug therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Systemic antimicrobial drug therapy seems to prevent UTIs , but primarily for patients catheterized for 3 to 14 days .
	manualset3
225577	2	421038	7	NULL	NULL	0	NULL	UTIs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Systemic antimicrobial drug therapy seems to prevent UTIs , but primarily for patients catheterized for 3 to 14 days .
	manualset3
225578	3	421038	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Systemic antimicrobial drug therapy seems to prevent UTIs , but primarily for patients catheterized for 3 to 14 days .
	manualset3
225579	4	421038	7	NULL	NULL	0	NULL	3 to 14 days 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Systemic antimicrobial drug therapy seems to prevent UTIs , but primarily for patients catheterized for 3 to 14 days .
	manualset3
225580	1	421039	7	NULL	NULL	0	NULL	Two stretches 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Two stretches of sequence upstream of pilE were devoid of transposon insertions , and some deletions in these regions were not recoverable , suggesting that they are essential for gonococcal viability .
	manualset3
225581	2	421039	7	NULL	NULL	0	NULL	sequence upstream	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Two stretches of sequence upstream of pilE were devoid of transposon insertions , and some deletions in these regions were not recoverable , suggesting that they are essential for gonococcal viability .
	manualset3
225582	3	421039	7	NULL	NULL	0	NULL	pilE	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Two stretches of sequence upstream of pilE were devoid of transposon insertions , and some deletions in these regions were not recoverable , suggesting that they are essential for gonococcal viability .
	manualset3
225583	4	421039	7	NULL	NULL	0	NULL	transposon insertions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two stretches of sequence upstream of pilE were devoid of transposon insertions , and some deletions in these regions were not recoverable , suggesting that they are essential for gonococcal viability .
	manualset3
225584	5	421039	7	NULL	NULL	0	NULL	deletions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two stretches of sequence upstream of pilE were devoid of transposon insertions , and some deletions in these regions were not recoverable , suggesting that they are essential for gonococcal viability .
	manualset3
225585	6	421039	7	NULL	NULL	0	NULL	regions	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Two stretches of sequence upstream of pilE were devoid of transposon insertions , and some deletions in these regions were not recoverable , suggesting that they are essential for gonococcal viability .
	manualset3
225586	7	421039	7	NULL	NULL	0	NULL	gonococcal viability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two stretches of sequence upstream of pilE were devoid of transposon insertions , and some deletions in these regions were not recoverable , suggesting that they are essential for gonococcal viability .
	manualset3
225587	1	421040	7	NULL	NULL	0	NULL	 greater incidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They were found to have a greater incidence of the standard atopic disorders -- asthma , eczema , recurrent urticaria , and hay fever .
	manualset3
225588	2	421040	7	NULL	NULL	0	NULL	standard atopic disorders 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	They were found to have a greater incidence of the standard atopic disorders -- asthma , eczema , recurrent urticaria , and hay fever .
	manualset3
225589	3	421040	7	NULL	NULL	0	NULL	asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	They were found to have a greater incidence of the standard atopic disorders -- asthma , eczema , recurrent urticaria , and hay fever .
	manualset3
225590	4	421040	7	NULL	NULL	0	NULL	eczema	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	They were found to have a greater incidence of the standard atopic disorders -- asthma , eczema , recurrent urticaria , and hay fever .
	manualset3
225591	5	421040	7	NULL	NULL	0	NULL	 recurrent urticaria	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	They were found to have a greater incidence of the standard atopic disorders -- asthma , eczema , recurrent urticaria , and hay fever .
	manualset3
225592	6	421040	7	NULL	NULL	0	NULL	hay fever	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	They were found to have a greater incidence of the standard atopic disorders -- asthma , eczema , recurrent urticaria , and hay fever .
	manualset3
225593	1	421041	7	NULL	NULL	0	NULL	 Survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Survival of patients with triple-vessel stenosing coronary atheroma ) .
	manualset3
225594	2	421041	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Survival of patients with triple-vessel stenosing coronary atheroma ) .
	manualset3
225595	3	421041	7	NULL	NULL	0	NULL	triple-vessel stenosing coronary atheroma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Survival of patients with triple-vessel stenosing coronary atheroma ) .
	manualset3
225596	1	421042	7	NULL	NULL	0	NULL	S-NO-albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	S-NO-albumin produced dose-dependent hypotension that was significantly augmented by prior infusion of either LMW thiol .
	manualset3
225597	2	421042	7	NULL	NULL	0	NULL	dose-dependent hypotension 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	S-NO-albumin produced dose-dependent hypotension that was significantly augmented by prior infusion of either LMW thiol .
	manualset3
225598	3	421042	7	NULL	NULL	0	NULL	infusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	S-NO-albumin produced dose-dependent hypotension that was significantly augmented by prior infusion of either LMW thiol .
	manualset3
225599	4	421042	7	NULL	NULL	0	NULL	LMW thiol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	S-NO-albumin produced dose-dependent hypotension that was significantly augmented by prior infusion of either LMW thiol .
	manualset3
225600	1	421043	7	NULL	NULL	0	NULL	mill streams	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the various mill streams , the last break and reduction streams produced lower quality bread and must be eliminated in milling .
	manualset3
225601	2	421043	7	NULL	NULL	0	NULL	last break	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the various mill streams , the last break and reduction streams produced lower quality bread and must be eliminated in milling .
	manualset3
225602	3	421043	7	NULL	NULL	0	NULL	reduction streams	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the various mill streams , the last break and reduction streams produced lower quality bread and must be eliminated in milling .
	manualset3
225603	4	421043	7	NULL	NULL	0	NULL	lower quality bread	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the various mill streams , the last break and reduction streams produced lower quality bread and must be eliminated in milling .
	manualset3
225604	5	421043	7	NULL	NULL	0	NULL	 milling 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the various mill streams , the last break and reduction streams produced lower quality bread and must be eliminated in milling .
	manualset3
225605	1	421044	7	NULL	NULL	0	NULL	positive regulators	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Among positive regulators , jasmonic acid ( JA ) accumulates in senescing leaves and the JA-insensitive coi1-1 mutant displays delayed leaf senescence in Arabidopsis .
	manualset3
225606	2	421044	7	NULL	NULL	0	NULL	 jasmonic acid ( JA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Among positive regulators , jasmonic acid ( JA ) accumulates in senescing leaves and the JA-insensitive coi1-1 mutant displays delayed leaf senescence in Arabidopsis .
	manualset3
225607	3	421044	7	NULL	NULL	0	NULL	senescing leaves	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Among positive regulators , jasmonic acid ( JA ) accumulates in senescing leaves and the JA-insensitive coi1-1 mutant displays delayed leaf senescence in Arabidopsis .
	manualset3
225608	4	421044	7	NULL	NULL	NULL	NULL	JA-insensitive coi1-1 mutant	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Among positive regulators , jasmonic acid ( JA ) accumulates in senescing leaves and the JA-insensitive coi1-1 mutant displays delayed leaf senescence in Arabidopsis .
	manualset3
225609	5	421044	7	NULL	NULL	0	NULL	delayed leaf senescence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among positive regulators , jasmonic acid ( JA ) accumulates in senescing leaves and the JA-insensitive coi1-1 mutant displays delayed leaf senescence in Arabidopsis .
	manualset3
225610	6	421044	7	NULL	NULL	0	NULL	Arabidopsis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Among positive regulators , jasmonic acid ( JA ) accumulates in senescing leaves and the JA-insensitive coi1-1 mutant displays delayed leaf senescence in Arabidopsis .
	manualset3
225611	1	421045	7	NULL	NULL	0	NULL	Inbreeding	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inbreeding and genetic structure in the endangered Sorraia horse breed : implications for its conservation and management .
	manualset3
225612	2	421045	7	NULL	NULL	0	NULL	 genetic structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Inbreeding and genetic structure in the endangered Sorraia horse breed : implications for its conservation and management .
	manualset3
225613	3	421045	7	NULL	NULL	0	NULL	endangered Sorraia horse breed	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Inbreeding and genetic structure in the endangered Sorraia horse breed : implications for its conservation and management .
	manualset3
225614	4	421045	7	NULL	NULL	0	NULL	implications	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inbreeding and genetic structure in the endangered Sorraia horse breed : implications for its conservation and management .
	manualset3
225615	5	421045	7	NULL	NULL	0	NULL	conservation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inbreeding and genetic structure in the endangered Sorraia horse breed : implications for its conservation and management .
	manualset3
225616	6	421045	7	NULL	NULL	0	NULL	 management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Inbreeding and genetic structure in the endangered Sorraia horse breed : implications for its conservation and management .
	manualset3
225617	1	421046	7	NULL	NULL	0	NULL	Hemolymph ion regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemolymph ion regulation and kinetic characteristics of the gill ( Na ( + ) , K ( + ) ) - ATPase in the hermit crab Clibanarius vittatus ( Decapoda , Anomura ) acclimated to high salinity .
	manualset3
225618	2	421046	7	NULL	NULL	NULL	NULL	kinetic characteristics	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Hemolymph ion regulation and kinetic characteristics of the gill ( Na ( + ) , K ( + ) ) - ATPase in the hermit crab Clibanarius vittatus ( Decapoda , Anomura ) acclimated to high salinity .
	manualset3
225619	3	421046	7	NULL	NULL	0	NULL	 gill	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemolymph ion regulation and kinetic characteristics of the gill ( Na ( + ) , K ( + ) ) - ATPase in the hermit crab Clibanarius vittatus ( Decapoda , Anomura ) acclimated to high salinity .
	manualset3
225620	4	421046	7	NULL	NULL	0	NULL	( Na ( + ) , K ( + ) ) - ATPase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemolymph ion regulation and kinetic characteristics of the gill ( Na ( + ) , K ( + ) ) - ATPase in the hermit crab Clibanarius vittatus ( Decapoda , Anomura ) acclimated to high salinity .
	manualset3
225621	5	421046	7	NULL	NULL	0	NULL	hermit crab	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemolymph ion regulation and kinetic characteristics of the gill ( Na ( + ) , K ( + ) ) - ATPase in the hermit crab Clibanarius vittatus ( Decapoda , Anomura ) acclimated to high salinity .
	manualset3
225622	6	421046	7	NULL	NULL	0	NULL	Clibanarius vittatus ( Decapoda , Anomura )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemolymph ion regulation and kinetic characteristics of the gill ( Na ( + ) , K ( + ) ) - ATPase in the hermit crab Clibanarius vittatus ( Decapoda , Anomura ) acclimated to high salinity .
	manualset3
225623	7	421046	7	NULL	NULL	0	NULL	high salinity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Hemolymph ion regulation and kinetic characteristics of the gill ( Na ( + ) , K ( + ) ) - ATPase in the hermit crab Clibanarius vittatus ( Decapoda , Anomura ) acclimated to high salinity .
	manualset3
225624	1	421047	7	NULL	NULL	0	NULL	 measurement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We also describe the measurement of the role of laser-induced molecular alignment on the dipole force in optical Stark deceleration and outline progress towards the realisation of chirped optical Stark deceleration for producing slow molecular beams with mK energy spreads .
	manualset3
225625	2	421047	7	NULL	NULL	NULL	NULL	role	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We also describe the measurement of the role of laser-induced molecular alignment on the dipole force in optical Stark deceleration and outline progress towards the realisation of chirped optical Stark deceleration for producing slow molecular beams with mK energy spreads .
	manualset3
225626	3	421047	7	NULL	NULL	0	NULL	 laser-induced molecular alignment 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We also describe the measurement of the role of laser-induced molecular alignment on the dipole force in optical Stark deceleration and outline progress towards the realisation of chirped optical Stark deceleration for producing slow molecular beams with mK energy spreads .
	manualset3
225627	4	421047	7	NULL	NULL	0	NULL	dipole force	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We also describe the measurement of the role of laser-induced molecular alignment on the dipole force in optical Stark deceleration and outline progress towards the realisation of chirped optical Stark deceleration for producing slow molecular beams with mK energy spreads .
	manualset3
225628	5	421047	7	NULL	NULL	0	NULL	optical Stark deceleration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We also describe the measurement of the role of laser-induced molecular alignment on the dipole force in optical Stark deceleration and outline progress towards the realisation of chirped optical Stark deceleration for producing slow molecular beams with mK energy spreads .
	manualset3
225629	6	421047	7	NULL	NULL	0	NULL	outline progress	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We also describe the measurement of the role of laser-induced molecular alignment on the dipole force in optical Stark deceleration and outline progress towards the realisation of chirped optical Stark deceleration for producing slow molecular beams with mK energy spreads .
	manualset3
225630	7	421047	7	NULL	NULL	0	NULL	realisation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We also describe the measurement of the role of laser-induced molecular alignment on the dipole force in optical Stark deceleration and outline progress towards the realisation of chirped optical Stark deceleration for producing slow molecular beams with mK energy spreads .
	manualset3
225631	8	421047	7	NULL	NULL	0	NULL	chirped optical Stark deceleration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We also describe the measurement of the role of laser-induced molecular alignment on the dipole force in optical Stark deceleration and outline progress towards the realisation of chirped optical Stark deceleration for producing slow molecular beams with mK energy spreads .
	manualset3
225632	9	421047	7	NULL	NULL	0	NULL	slow molecular beams	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We also describe the measurement of the role of laser-induced molecular alignment on the dipole force in optical Stark deceleration and outline progress towards the realisation of chirped optical Stark deceleration for producing slow molecular beams with mK energy spreads .
	manualset3
225633	10	421047	7	NULL	NULL	0	NULL	mK energy spreads	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We also describe the measurement of the role of laser-induced molecular alignment on the dipole force in optical Stark deceleration and outline progress towards the realisation of chirped optical Stark deceleration for producing slow molecular beams with mK energy spreads .
	manualset3
225634	1	421048	7	NULL	NULL	0	NULL	Attachment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Attachment to thermistors may limit the range of movement and comfort , introducing a potential confound that may prolong sleep initiation or increase wakefulness after sleep onset .
	manualset3
225635	2	421048	7	NULL	NULL	0	NULL	thermistors	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Attachment to thermistors may limit the range of movement and comfort , introducing a potential confound that may prolong sleep initiation or increase wakefulness after sleep onset .
	manualset3
225636	3	421048	7	NULL	NULL	0	NULL	 range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Attachment to thermistors may limit the range of movement and comfort , introducing a potential confound that may prolong sleep initiation or increase wakefulness after sleep onset .
	manualset3
225637	4	421048	7	NULL	NULL	0	NULL	movement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Attachment to thermistors may limit the range of movement and comfort , introducing a potential confound that may prolong sleep initiation or increase wakefulness after sleep onset .
	manualset3
225638	5	421048	7	NULL	NULL	0	NULL	comfort	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Attachment to thermistors may limit the range of movement and comfort , introducing a potential confound that may prolong sleep initiation or increase wakefulness after sleep onset .
	manualset3
225639	6	421048	7	NULL	NULL	0	NULL	potential confound	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Attachment to thermistors may limit the range of movement and comfort , introducing a potential confound that may prolong sleep initiation or increase wakefulness after sleep onset .
	manualset3
225640	7	421048	7	NULL	NULL	0	NULL	sleep initiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Attachment to thermistors may limit the range of movement and comfort , introducing a potential confound that may prolong sleep initiation or increase wakefulness after sleep onset .
	manualset3
225641	8	421048	7	NULL	NULL	0	NULL	 wakefulness	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Attachment to thermistors may limit the range of movement and comfort , introducing a potential confound that may prolong sleep initiation or increase wakefulness after sleep onset .
	manualset3
225642	9	421048	7	NULL	NULL	0	NULL	sleep onset	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Attachment to thermistors may limit the range of movement and comfort , introducing a potential confound that may prolong sleep initiation or increase wakefulness after sleep onset .
	manualset3
225643	1	421049	7	NULL	NULL	0	NULL	algorithm 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The algorithm uses correlation of temporal features across space , and therefore differs from conventional optical flow algorithms which use correlation of spatial features over time .
	manualset3
225644	2	421049	7	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The algorithm uses correlation of temporal features across space , and therefore differs from conventional optical flow algorithms which use correlation of spatial features over time .
	manualset3
225645	3	421049	7	NULL	NULL	0	NULL	temporal features	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The algorithm uses correlation of temporal features across space , and therefore differs from conventional optical flow algorithms which use correlation of spatial features over time .
	manualset3
225646	4	421049	7	NULL	NULL	0	NULL	space	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The algorithm uses correlation of temporal features across space , and therefore differs from conventional optical flow algorithms which use correlation of spatial features over time .
	manualset3
225647	5	421049	7	NULL	NULL	0	NULL	conventional optical flow algorithms	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The algorithm uses correlation of temporal features across space , and therefore differs from conventional optical flow algorithms which use correlation of spatial features over time .
	manualset3
225648	6	421049	7	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The algorithm uses correlation of temporal features across space , and therefore differs from conventional optical flow algorithms which use correlation of spatial features over time .
	manualset3
225649	7	421049	7	NULL	NULL	0	NULL	spatial features 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The algorithm uses correlation of temporal features across space , and therefore differs from conventional optical flow algorithms which use correlation of spatial features over time .
	manualset3
225650	8	421049	7	NULL	NULL	0	NULL	 time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The algorithm uses correlation of temporal features across space , and therefore differs from conventional optical flow algorithms which use correlation of spatial features over time .
	manualset3
225651	1	421050	7	NULL	NULL	0	NULL	 Determination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of blood mucoproteins & the Kunkelphenol reaction in the etiological diagnosis of icterus & the functional examination of the liver in general ) .
	manualset3
225652	2	421050	7	NULL	NULL	0	NULL	blood mucoproteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of blood mucoproteins & the Kunkelphenol reaction in the etiological diagnosis of icterus & the functional examination of the liver in general ) .
	manualset3
225653	3	421050	7	NULL	NULL	0	NULL	Kunkelphenol reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of blood mucoproteins & the Kunkelphenol reaction in the etiological diagnosis of icterus & the functional examination of the liver in general ) .
	manualset3
225654	4	421050	7	NULL	NULL	0	NULL	 etiological diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of blood mucoproteins & the Kunkelphenol reaction in the etiological diagnosis of icterus & the functional examination of the liver in general ) .
	manualset3
225655	5	421050	7	NULL	NULL	0	NULL	icterus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of blood mucoproteins & the Kunkelphenol reaction in the etiological diagnosis of icterus & the functional examination of the liver in general ) .
	manualset3
225656	6	421050	7	NULL	NULL	0	NULL	functional examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of blood mucoproteins & the Kunkelphenol reaction in the etiological diagnosis of icterus & the functional examination of the liver in general ) .
	manualset3
225657	7	421050	7	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of blood mucoproteins & the Kunkelphenol reaction in the etiological diagnosis of icterus & the functional examination of the liver in general ) .
	manualset3
225658	1	421051	7	NULL	NULL	0	NULL	3 - ( 7-methylimidazo ( 1 , 2-b ) pyridazin-6-yl ) oxy-2 , 2 - dimethylpropanesulfonamide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Among them , 3 - ( 7-methylimidazo ( 1 , 2-b ) pyridazin-6-yl ) oxy-2 , 2 - dimethylpropanesulfonamide ( 25 ) showed the most potent inhibitory effect , and its anti-asthmatic effect in an experimental model of allergic asthma was superior to that of theophylline .
	manualset3
225659	2	421051	7	NULL	NULL	0	NULL	potent inhibitory effect 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among them , 3 - ( 7-methylimidazo ( 1 , 2-b ) pyridazin-6-yl ) oxy-2 , 2 - dimethylpropanesulfonamide ( 25 ) showed the most potent inhibitory effect , and its anti-asthmatic effect in an experimental model of allergic asthma was superior to that of theophylline .
	manualset3
225660	3	421051	7	NULL	NULL	0	NULL	anti-asthmatic effect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among them , 3 - ( 7-methylimidazo ( 1 , 2-b ) pyridazin-6-yl ) oxy-2 , 2 - dimethylpropanesulfonamide ( 25 ) showed the most potent inhibitory effect , and its anti-asthmatic effect in an experimental model of allergic asthma was superior to that of theophylline .
	manualset3
225661	4	421051	7	NULL	NULL	0	NULL	experimental model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Among them , 3 - ( 7-methylimidazo ( 1 , 2-b ) pyridazin-6-yl ) oxy-2 , 2 - dimethylpropanesulfonamide ( 25 ) showed the most potent inhibitory effect , and its anti-asthmatic effect in an experimental model of allergic asthma was superior to that of theophylline .
	manualset3
225662	5	421051	7	NULL	NULL	0	NULL	allergic asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Among them , 3 - ( 7-methylimidazo ( 1 , 2-b ) pyridazin-6-yl ) oxy-2 , 2 - dimethylpropanesulfonamide ( 25 ) showed the most potent inhibitory effect , and its anti-asthmatic effect in an experimental model of allergic asthma was superior to that of theophylline .
	manualset3
225663	6	421051	7	NULL	NULL	0	NULL	 theophylline	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Among them , 3 - ( 7-methylimidazo ( 1 , 2-b ) pyridazin-6-yl ) oxy-2 , 2 - dimethylpropanesulfonamide ( 25 ) showed the most potent inhibitory effect , and its anti-asthmatic effect in an experimental model of allergic asthma was superior to that of theophylline .
	manualset3
225664	1	421052	7	NULL	NULL	0	NULL	experiments 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In both experiments , in all lighting conditions we found higher plasma levels of LH and FSH during the dark than the light period .
	manualset3
225665	2	421052	7	NULL	NULL	0	NULL	lighting conditions 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In both experiments , in all lighting conditions we found higher plasma levels of LH and FSH during the dark than the light period .
	manualset3
225666	3	421052	7	NULL	NULL	0	NULL	higher plasma levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In both experiments , in all lighting conditions we found higher plasma levels of LH and FSH during the dark than the light period .
	manualset3
225667	4	421052	7	NULL	NULL	0	NULL	LH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In both experiments , in all lighting conditions we found higher plasma levels of LH and FSH during the dark than the light period .
	manualset3
225668	5	421052	7	NULL	NULL	0	NULL	FSH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In both experiments , in all lighting conditions we found higher plasma levels of LH and FSH during the dark than the light period .
	manualset3
225669	6	421052	7	NULL	NULL	0	NULL	dark period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In both experiments , in all lighting conditions we found higher plasma levels of LH and FSH during the dark than the light period .
	manualset3
225670	7	421052	7	NULL	NULL	0	NULL	 light period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In both experiments , in all lighting conditions we found higher plasma levels of LH and FSH during the dark than the light period .
	manualset3
225671	1	421053	7	NULL	NULL	0	NULL	Single amino acid substitutions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Single amino acid substitutions , including a conserved Lys residue in the center of the putative TMD , did not affect TAP2 expression levels .
	manualset3
225672	2	421053	7	NULL	NULL	0	NULL	conserved Lys residue	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Single amino acid substitutions , including a conserved Lys residue in the center of the putative TMD , did not affect TAP2 expression levels .
	manualset3
225673	3	421053	7	NULL	NULL	0	NULL	center of the putative TMD	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Single amino acid substitutions , including a conserved Lys residue in the center of the putative TMD , did not affect TAP2 expression levels .
	manualset3
225674	4	421053	7	NULL	NULL	0	NULL	TAP2 expression levels	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Single amino acid substitutions , including a conserved Lys residue in the center of the putative TMD , did not affect TAP2 expression levels .
	manualset3
225675	1	421054	7	NULL	NULL	0	NULL	Evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluation of atrazine removal processes in a wetland .
	manualset3
225676	2	421054	7	NULL	NULL	0	NULL	atrazine removal processes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluation of atrazine removal processes in a wetland .
	manualset3
225677	3	421054	7	NULL	NULL	0	NULL	wetland	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluation of atrazine removal processes in a wetland .
	manualset3
225678	1	421055	7	NULL	NULL	0	NULL	hsps 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Like the hsps , Osp94 has a putative amino-terminal ATP-binding domain and a putative carboxyl-terminal peptide-binding domain .
	manualset3
225679	2	421055	7	NULL	NULL	0	NULL	Osp94 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Like the hsps , Osp94 has a putative amino-terminal ATP-binding domain and a putative carboxyl-terminal peptide-binding domain .
	manualset3
225680	3	421055	7	NULL	NULL	0	NULL	putative amino-terminal ATP-binding domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Like the hsps , Osp94 has a putative amino-terminal ATP-binding domain and a putative carboxyl-terminal peptide-binding domain .
	manualset3
225681	4	421055	7	NULL	NULL	0	NULL	putative carboxyl-terminal peptide-binding domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Like the hsps , Osp94 has a putative amino-terminal ATP-binding domain and a putative carboxyl-terminal peptide-binding domain .
	manualset3
225682	1	421056	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results at least partially explain the discrepancy between published HPMS data and earlier FT-ICR findings and call for the utmost care in using FT-ICR for gas-phase basicity measurements of heavily fluorinated compounds .
	manualset3
225683	2	421056	7	NULL	NULL	0	NULL	discrepancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results at least partially explain the discrepancy between published HPMS data and earlier FT-ICR findings and call for the utmost care in using FT-ICR for gas-phase basicity measurements of heavily fluorinated compounds .
	manualset3
225684	3	421056	7	NULL	NULL	0	NULL	 published HPMS data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These results at least partially explain the discrepancy between published HPMS data and earlier FT-ICR findings and call for the utmost care in using FT-ICR for gas-phase basicity measurements of heavily fluorinated compounds .
	manualset3
225685	4	421056	7	NULL	NULL	0	NULL	FT-ICR findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results at least partially explain the discrepancy between published HPMS data and earlier FT-ICR findings and call for the utmost care in using FT-ICR for gas-phase basicity measurements of heavily fluorinated compounds .
	manualset3
225686	5	421056	7	NULL	NULL	0	NULL	call	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results at least partially explain the discrepancy between published HPMS data and earlier FT-ICR findings and call for the utmost care in using FT-ICR for gas-phase basicity measurements of heavily fluorinated compounds .
	manualset3
225687	6	421056	7	NULL	NULL	0	NULL	utmost care	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results at least partially explain the discrepancy between published HPMS data and earlier FT-ICR findings and call for the utmost care in using FT-ICR for gas-phase basicity measurements of heavily fluorinated compounds .
	manualset3
225688	7	421056	7	NULL	NULL	0	NULL	 FT-ICR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These results at least partially explain the discrepancy between published HPMS data and earlier FT-ICR findings and call for the utmost care in using FT-ICR for gas-phase basicity measurements of heavily fluorinated compounds .
	manualset3
225689	8	421056	7	NULL	NULL	0	NULL	gas-phase basicity measurements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results at least partially explain the discrepancy between published HPMS data and earlier FT-ICR findings and call for the utmost care in using FT-ICR for gas-phase basicity measurements of heavily fluorinated compounds .
	manualset3
225690	9	421056	7	NULL	NULL	0	NULL	heavily fluorinated compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These results at least partially explain the discrepancy between published HPMS data and earlier FT-ICR findings and call for the utmost care in using FT-ICR for gas-phase basicity measurements of heavily fluorinated compounds .
	manualset3
225691	1	421057	7	NULL	NULL	0	NULL	Beneficial effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Beneficial effects of propolis on human health and neurological diseases .
	manualset3
225692	2	421057	7	NULL	NULL	0	NULL	propolis 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Beneficial effects of propolis on human health and neurological diseases .
	manualset3
225693	3	421057	7	NULL	NULL	0	NULL	human health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Beneficial effects of propolis on human health and neurological diseases .
	manualset3
225694	4	421057	7	NULL	NULL	0	NULL	 neurological diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Beneficial effects of propolis on human health and neurological diseases .
	manualset3
225695	1	421058	7	NULL	NULL	0	NULL	 cumulative experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cumulative experience from these studies have demonstrated an advantageous effect on postoperative morbidity parameters such as blood loss , postoperative thromboembolic complications , pulmonary infective complications , gastrointestinal motility , postoperative hospital stay , etc. .
	manualset3
225696	2	421058	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cumulative experience from these studies have demonstrated an advantageous effect on postoperative morbidity parameters such as blood loss , postoperative thromboembolic complications , pulmonary infective complications , gastrointestinal motility , postoperative hospital stay , etc. .
	manualset3
225697	3	421058	7	NULL	NULL	0	NULL	advantageous effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cumulative experience from these studies have demonstrated an advantageous effect on postoperative morbidity parameters such as blood loss , postoperative thromboembolic complications , pulmonary infective complications , gastrointestinal motility , postoperative hospital stay , etc. .
	manualset3
225698	4	421058	7	NULL	NULL	NULL	NULL	postoperative morbidity parameters	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The cumulative experience from these studies have demonstrated an advantageous effect on postoperative morbidity parameters such as blood loss , postoperative thromboembolic complications , pulmonary infective complications , gastrointestinal motility , postoperative hospital stay , etc. .
	manualset3
225699	5	421058	7	NULL	NULL	0	NULL	blood loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cumulative experience from these studies have demonstrated an advantageous effect on postoperative morbidity parameters such as blood loss , postoperative thromboembolic complications , pulmonary infective complications , gastrointestinal motility , postoperative hospital stay , etc. .
	manualset3
225700	6	421058	7	NULL	NULL	0	NULL	postoperative thromboembolic complications 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cumulative experience from these studies have demonstrated an advantageous effect on postoperative morbidity parameters such as blood loss , postoperative thromboembolic complications , pulmonary infective complications , gastrointestinal motility , postoperative hospital stay , etc. .
	manualset3
225701	7	421058	7	NULL	NULL	0	NULL	 pulmonary infective complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cumulative experience from these studies have demonstrated an advantageous effect on postoperative morbidity parameters such as blood loss , postoperative thromboembolic complications , pulmonary infective complications , gastrointestinal motility , postoperative hospital stay , etc. .
	manualset3
225702	8	421058	7	NULL	NULL	0	NULL	gastrointestinal motility	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cumulative experience from these studies have demonstrated an advantageous effect on postoperative morbidity parameters such as blood loss , postoperative thromboembolic complications , pulmonary infective complications , gastrointestinal motility , postoperative hospital stay , etc. .
	manualset3
225703	9	421058	7	NULL	NULL	0	NULL	postoperative hospital stay	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cumulative experience from these studies have demonstrated an advantageous effect on postoperative morbidity parameters such as blood loss , postoperative thromboembolic complications , pulmonary infective complications , gastrointestinal motility , postoperative hospital stay , etc. .
	manualset3
225704	1	421059	7	NULL	NULL	0	NULL	Maximal suppression 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal suppression of proliferation of spleen cells in response to ConA and TLA was observed on days 7 and 14 after infection and correlated with elevated levels of nitrite in spleen cell culture supernatants .
	manualset3
225705	2	421059	7	NULL	NULL	0	NULL	proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal suppression of proliferation of spleen cells in response to ConA and TLA was observed on days 7 and 14 after infection and correlated with elevated levels of nitrite in spleen cell culture supernatants .
	manualset3
225706	3	421059	7	NULL	NULL	0	NULL	spleen cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal suppression of proliferation of spleen cells in response to ConA and TLA was observed on days 7 and 14 after infection and correlated with elevated levels of nitrite in spleen cell culture supernatants .
	manualset3
225707	4	421059	7	NULL	NULL	0	NULL	response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal suppression of proliferation of spleen cells in response to ConA and TLA was observed on days 7 and 14 after infection and correlated with elevated levels of nitrite in spleen cell culture supernatants .
	manualset3
225708	5	421059	7	NULL	NULL	0	NULL	ConA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal suppression of proliferation of spleen cells in response to ConA and TLA was observed on days 7 and 14 after infection and correlated with elevated levels of nitrite in spleen cell culture supernatants .
	manualset3
225709	6	421059	7	NULL	NULL	0	NULL	 TLA 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal suppression of proliferation of spleen cells in response to ConA and TLA was observed on days 7 and 14 after infection and correlated with elevated levels of nitrite in spleen cell culture supernatants .
	manualset3
225710	7	421059	7	NULL	NULL	0	NULL	days 7 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal suppression of proliferation of spleen cells in response to ConA and TLA was observed on days 7 and 14 after infection and correlated with elevated levels of nitrite in spleen cell culture supernatants .
	manualset3
225711	8	421059	7	NULL	NULL	0	NULL	14	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal suppression of proliferation of spleen cells in response to ConA and TLA was observed on days 7 and 14 after infection and correlated with elevated levels of nitrite in spleen cell culture supernatants .
	manualset3
225712	9	421059	7	NULL	NULL	0	NULL	infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal suppression of proliferation of spleen cells in response to ConA and TLA was observed on days 7 and 14 after infection and correlated with elevated levels of nitrite in spleen cell culture supernatants .
	manualset3
225713	10	421059	7	NULL	NULL	0	NULL	elevated levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal suppression of proliferation of spleen cells in response to ConA and TLA was observed on days 7 and 14 after infection and correlated with elevated levels of nitrite in spleen cell culture supernatants .
	manualset3
225714	11	421059	7	NULL	NULL	0	NULL	nitrite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal suppression of proliferation of spleen cells in response to ConA and TLA was observed on days 7 and 14 after infection and correlated with elevated levels of nitrite in spleen cell culture supernatants .
	manualset3
225715	12	421059	7	NULL	NULL	0	NULL	spleen cell culture supernatants	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Maximal suppression of proliferation of spleen cells in response to ConA and TLA was observed on days 7 and 14 after infection and correlated with elevated levels of nitrite in spleen cell culture supernatants .
	manualset3
225716	1	421060	7	NULL	NULL	0	NULL	93	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Among them , 93 had strictly defined severe malaria , and 95 had less severe malaria .
	manualset3
225717	2	421060	7	NULL	NULL	0	NULL	severe malaria	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Among them , 93 had strictly defined severe malaria , and 95 had less severe malaria .
	manualset3
225718	3	421060	7	NULL	NULL	0	NULL	 95	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Among them , 93 had strictly defined severe malaria , and 95 had less severe malaria .
	manualset3
225719	4	421060	7	NULL	NULL	0	NULL	less severe malaria	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Among them , 93 had strictly defined severe malaria , and 95 had less severe malaria .
	manualset3
225720	1	421061	7	NULL	NULL	0	NULL	Retinal fluorescein angiography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinal fluorescein and indocyanine green angiography and spectral-domain optical coherence tomography findings in acute retinal pigment epitheliitis .
	manualset3
225721	2	421061	7	NULL	NULL	0	NULL	indocyanine green angiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinal fluorescein and indocyanine green angiography and spectral-domain optical coherence tomography findings in acute retinal pigment epitheliitis .
	manualset3
225722	3	421061	7	NULL	NULL	0	NULL	spectral-domain optical coherence tomography findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinal fluorescein and indocyanine green angiography and spectral-domain optical coherence tomography findings in acute retinal pigment epitheliitis .
	manualset3
225723	4	421061	7	NULL	NULL	0	NULL	acute retinal pigment epitheliitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Retinal fluorescein and indocyanine green angiography and spectral-domain optical coherence tomography findings in acute retinal pigment epitheliitis .
	manualset3
225724	1	421062	7	NULL	NULL	0	NULL	Breathing pattern	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Breathing pattern was described by the equation VE = M ( VT - K ) and the response to carbon dioxide by VE = S ( PCO2 - B ) .
	manualset3
225725	2	421062	7	NULL	NULL	0	NULL	 equation VE = M ( VT - K )	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Breathing pattern was described by the equation VE = M ( VT - K ) and the response to carbon dioxide by VE = S ( PCO2 - B ) .
	manualset3
225726	3	421062	7	NULL	NULL	0	NULL	response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Breathing pattern was described by the equation VE = M ( VT - K ) and the response to carbon dioxide by VE = S ( PCO2 - B ) .
	manualset3
225727	4	421062	7	NULL	NULL	0	NULL	 carbon dioxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Breathing pattern was described by the equation VE = M ( VT - K ) and the response to carbon dioxide by VE = S ( PCO2 - B ) .
	manualset3
225728	5	421062	7	NULL	NULL	0	NULL	VE = S ( PCO2 - B )	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Breathing pattern was described by the equation VE = M ( VT - K ) and the response to carbon dioxide by VE = S ( PCO2 - B ) .
	manualset3
225729	1	421063	7	NULL	NULL	0	NULL	lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Both lesions were successfully treated by patch repair .
	manualset3
225730	2	421063	7	NULL	NULL	0	NULL	patch repair	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Both lesions were successfully treated by patch repair .
	manualset3
225731	1	421064	7	NULL	NULL	NULL	NULL	Increase	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Increase of heat shock protein gene expression by melatonin in AR42J cells .
	manualset3
225732	2	421064	7	NULL	NULL	0	NULL	heat shock protein gene expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increase of heat shock protein gene expression by melatonin in AR42J cells .
	manualset3
225733	3	421064	7	NULL	NULL	0	NULL	melatonin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Increase of heat shock protein gene expression by melatonin in AR42J cells .
	manualset3
225734	4	421064	7	NULL	NULL	0	NULL	AR42J cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Increase of heat shock protein gene expression by melatonin in AR42J cells .
	manualset3
225735	1	421065	7	NULL	NULL	0	NULL	Estimation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Estimation of local oxygen transmissibilities suggests that a Dk/L & lt ; 3 x 10 ( -9 ) may produce this gross clinical sign underneath the lens midperiphery , whereas central Dk/L ) or = 6 x 10 ( -9 ) may be sufficient to prevent its appearance .
	manualset3
225736	2	421065	7	NULL	NULL	0	NULL	local oxygen transmissibilities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Estimation of local oxygen transmissibilities suggests that a Dk/L & lt ; 3 x 10 ( -9 ) may produce this gross clinical sign underneath the lens midperiphery , whereas central Dk/L ) or = 6 x 10 ( -9 ) may be sufficient to prevent its appearance .
	manualset3
225737	3	421065	7	NULL	NULL	0	NULL	Dk/L & lt	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Estimation of local oxygen transmissibilities suggests that a Dk/L & lt ; 3 x 10 ( -9 ) may produce this gross clinical sign underneath the lens midperiphery , whereas central Dk/L ) or = 6 x 10 ( -9 ) may be sufficient to prevent its appearance .
	manualset3
225738	4	421065	7	NULL	NULL	0	NULL	3 x 10 ( -9 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Estimation of local oxygen transmissibilities suggests that a Dk/L & lt ; 3 x 10 ( -9 ) may produce this gross clinical sign underneath the lens midperiphery , whereas central Dk/L ) or = 6 x 10 ( -9 ) may be sufficient to prevent its appearance .
	manualset3
225739	5	421065	7	NULL	NULL	0	NULL	gross clinical sign 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Estimation of local oxygen transmissibilities suggests that a Dk/L & lt ; 3 x 10 ( -9 ) may produce this gross clinical sign underneath the lens midperiphery , whereas central Dk/L ) or = 6 x 10 ( -9 ) may be sufficient to prevent its appearance .
	manualset3
225740	6	421065	7	NULL	NULL	0	NULL	lens midperiphery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Estimation of local oxygen transmissibilities suggests that a Dk/L & lt ; 3 x 10 ( -9 ) may produce this gross clinical sign underneath the lens midperiphery , whereas central Dk/L ) or = 6 x 10 ( -9 ) may be sufficient to prevent its appearance .
	manualset3
225741	7	421065	7	NULL	NULL	0	NULL	central Dk/L	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Estimation of local oxygen transmissibilities suggests that a Dk/L & lt ; 3 x 10 ( -9 ) may produce this gross clinical sign underneath the lens midperiphery , whereas central Dk/L ) or = 6 x 10 ( -9 ) may be sufficient to prevent its appearance .
	manualset3
225742	8	421065	7	NULL	NULL	0	NULL	6 x 10 ( -9 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Estimation of local oxygen transmissibilities suggests that a Dk/L & lt ; 3 x 10 ( -9 ) may produce this gross clinical sign underneath the lens midperiphery , whereas central Dk/L ) or = 6 x 10 ( -9 ) may be sufficient to prevent its appearance .
	manualset3
225743	9	421065	7	NULL	NULL	0	NULL	appearance 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Estimation of local oxygen transmissibilities suggests that a Dk/L & lt ; 3 x 10 ( -9 ) may produce this gross clinical sign underneath the lens midperiphery , whereas central Dk/L ) or = 6 x 10 ( -9 ) may be sufficient to prevent its appearance .
	manualset3
225744	1	421066	7	NULL	NULL	0	NULL	1986 to 1996	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	From 1986 to 1996 148 children underwent BMT , and are included in a retrospective analysis of the incidence , risk factors and outcome of IFI .
	manualset3
225745	2	421066	7	NULL	NULL	0	NULL	148 children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	From 1986 to 1996 148 children underwent BMT , and are included in a retrospective analysis of the incidence , risk factors and outcome of IFI .
	manualset3
225746	3	421066	7	NULL	NULL	0	NULL	BMT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	From 1986 to 1996 148 children underwent BMT , and are included in a retrospective analysis of the incidence , risk factors and outcome of IFI .
	manualset3
225747	4	421066	7	NULL	NULL	0	NULL	 retrospective analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	From 1986 to 1996 148 children underwent BMT , and are included in a retrospective analysis of the incidence , risk factors and outcome of IFI .
	manualset3
225748	5	421066	7	NULL	NULL	0	NULL	 incidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	From 1986 to 1996 148 children underwent BMT , and are included in a retrospective analysis of the incidence , risk factors and outcome of IFI .
	manualset3
225749	6	421066	7	NULL	NULL	0	NULL	 risk factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	From 1986 to 1996 148 children underwent BMT , and are included in a retrospective analysis of the incidence , risk factors and outcome of IFI .
	manualset3
225750	7	421066	7	NULL	NULL	0	NULL	outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	From 1986 to 1996 148 children underwent BMT , and are included in a retrospective analysis of the incidence , risk factors and outcome of IFI .
	manualset3
225751	8	421066	7	NULL	NULL	0	NULL	IFI	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	From 1986 to 1996 148 children underwent BMT , and are included in a retrospective analysis of the incidence , risk factors and outcome of IFI .
	manualset3
225752	1	421067	7	NULL	NULL	0	NULL	Delta133p53	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Among them , Delta133p53 lacks the 132 proximal residues and has been shown to modulate p53-induced apoptosis and cell-cycle arrest .
	manualset3
225753	2	421067	7	NULL	NULL	0	NULL	132 proximal residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Among them , Delta133p53 lacks the 132 proximal residues and has been shown to modulate p53-induced apoptosis and cell-cycle arrest .
	manualset3
225754	3	421067	7	NULL	NULL	0	NULL	p53-induced apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among them , Delta133p53 lacks the 132 proximal residues and has been shown to modulate p53-induced apoptosis and cell-cycle arrest .
	manualset3
225755	4	421067	7	NULL	NULL	0	NULL	cell-cycle arrest	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among them , Delta133p53 lacks the 132 proximal residues and has been shown to modulate p53-induced apoptosis and cell-cycle arrest .
	manualset3
225756	1	421068	7	NULL	NULL	0	NULL	Cost estimation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Cost estimation demonstrated that PT may be significantly more expensive than bedside OT .
	manualset3
225757	2	421068	7	NULL	NULL	0	NULL	PT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Cost estimation demonstrated that PT may be significantly more expensive than bedside OT .
	manualset3
225758	3	421068	7	NULL	NULL	0	NULL	bedside OT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Cost estimation demonstrated that PT may be significantly more expensive than bedside OT .
	manualset3
225759	1	421069	7	NULL	NULL	0	NULL	Trimethoprim/Sulfa	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Trimethoprim/Sulfa ( 72 % ) , ampicillin ( 64.5 % ) , enrofloxacin ( 55.3 % ) , and ciprofloxacin ( 47.4 % ) were the major antimicrobial resistance frequencies observed .
	manualset3
225760	2	421069	7	NULL	NULL	0	NULL	72 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Trimethoprim/Sulfa ( 72 % ) , ampicillin ( 64.5 % ) , enrofloxacin ( 55.3 % ) , and ciprofloxacin ( 47.4 % ) were the major antimicrobial resistance frequencies observed .
	manualset3
225761	3	421069	7	NULL	NULL	0	NULL	ampicillin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Trimethoprim/Sulfa ( 72 % ) , ampicillin ( 64.5 % ) , enrofloxacin ( 55.3 % ) , and ciprofloxacin ( 47.4 % ) were the major antimicrobial resistance frequencies observed .
	manualset3
225762	4	421069	7	NULL	NULL	0	NULL	64.5 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Trimethoprim/Sulfa ( 72 % ) , ampicillin ( 64.5 % ) , enrofloxacin ( 55.3 % ) , and ciprofloxacin ( 47.4 % ) were the major antimicrobial resistance frequencies observed .
	manualset3
225763	5	421069	7	NULL	NULL	0	NULL	 enrofloxacin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Trimethoprim/Sulfa ( 72 % ) , ampicillin ( 64.5 % ) , enrofloxacin ( 55.3 % ) , and ciprofloxacin ( 47.4 % ) were the major antimicrobial resistance frequencies observed .
	manualset3
225764	6	421069	7	NULL	NULL	0	NULL	55.3 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Trimethoprim/Sulfa ( 72 % ) , ampicillin ( 64.5 % ) , enrofloxacin ( 55.3 % ) , and ciprofloxacin ( 47.4 % ) were the major antimicrobial resistance frequencies observed .
	manualset3
225765	7	421069	7	NULL	NULL	0	NULL	ciprofloxacin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Trimethoprim/Sulfa ( 72 % ) , ampicillin ( 64.5 % ) , enrofloxacin ( 55.3 % ) , and ciprofloxacin ( 47.4 % ) were the major antimicrobial resistance frequencies observed .
	manualset3
225766	8	421069	7	NULL	NULL	0	NULL	47.4 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Trimethoprim/Sulfa ( 72 % ) , ampicillin ( 64.5 % ) , enrofloxacin ( 55.3 % ) , and ciprofloxacin ( 47.4 % ) were the major antimicrobial resistance frequencies observed .
	manualset3
225767	9	421069	7	NULL	NULL	0	NULL	antimicrobial resistance frequencies	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Trimethoprim/Sulfa ( 72 % ) , ampicillin ( 64.5 % ) , enrofloxacin ( 55.3 % ) , and ciprofloxacin ( 47.4 % ) were the major antimicrobial resistance frequencies observed .
	manualset3
225768	1	421070	7	NULL	NULL	0	NULL	angular tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The angular tissues showed similarities for most hydrolases with the exceptions of beta-Gal , UE , APM , APA and DPPIV .
	manualset3
225769	2	421070	7	NULL	NULL	0	NULL	similarities	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The angular tissues showed similarities for most hydrolases with the exceptions of beta-Gal , UE , APM , APA and DPPIV .
	manualset3
225770	3	421070	7	NULL	NULL	0	NULL	hydrolases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The angular tissues showed similarities for most hydrolases with the exceptions of beta-Gal , UE , APM , APA and DPPIV .
	manualset3
225771	4	421070	7	NULL	NULL	0	NULL	exceptions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The angular tissues showed similarities for most hydrolases with the exceptions of beta-Gal , UE , APM , APA and DPPIV .
	manualset3
225772	5	421070	7	NULL	NULL	NULL	NULL	 beta-Gal	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The angular tissues showed similarities for most hydrolases with the exceptions of beta-Gal , UE , APM , APA and DPPIV .
	manualset3
225773	6	421070	7	NULL	NULL	0	NULL	UE	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The angular tissues showed similarities for most hydrolases with the exceptions of beta-Gal , UE , APM , APA and DPPIV .
	manualset3
225774	7	421070	7	NULL	NULL	0	NULL	APM 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The angular tissues showed similarities for most hydrolases with the exceptions of beta-Gal , UE , APM , APA and DPPIV .
	manualset3
225775	8	421070	7	NULL	NULL	0	NULL	APA 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The angular tissues showed similarities for most hydrolases with the exceptions of beta-Gal , UE , APM , APA and DPPIV .
	manualset3
225776	9	421070	7	NULL	NULL	0	NULL	DPPIV	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The angular tissues showed similarities for most hydrolases with the exceptions of beta-Gal , UE , APM , APA and DPPIV .
	manualset3
225777	1	421071	7	NULL	NULL	0	NULL	novel microfluidic disk	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of a novel microfluidic disk in the analysis of single-cell viability and the application to Jurkat cells .
	manualset3
225778	2	421071	7	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of a novel microfluidic disk in the analysis of single-cell viability and the application to Jurkat cells .
	manualset3
225779	3	421071	7	NULL	NULL	NULL	NULL	single-cell viability	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of a novel microfluidic disk in the analysis of single-cell viability and the application to Jurkat cells .
	manualset3
225780	4	421071	7	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of a novel microfluidic disk in the analysis of single-cell viability and the application to Jurkat cells .
	manualset3
225781	5	421071	7	NULL	NULL	0	NULL	Jurkat cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of a novel microfluidic disk in the analysis of single-cell viability and the application to Jurkat cells .
	manualset3
225782	6	421071	7	NULL	NULL	0	NULL	Use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Use of a novel microfluidic disk in the analysis of single-cell viability and the application to Jurkat cells .
	manualset3
225783	1	421072	7	NULL	NULL	0	NULL	Thrombophlebitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Thrombophlebitis of the facial vein ) .
	manualset3
225784	2	421072	7	NULL	NULL	0	NULL	 facial vein 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Thrombophlebitis of the facial vein ) .
	manualset3
225785	1	421073	7	NULL	NULL	0	NULL	NMR investigation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR investigation of the futile cycling of ethanol in chronic alcoholic rats .
	manualset3
225786	2	421073	7	NULL	NULL	0	NULL	futile cycling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR investigation of the futile cycling of ethanol in chronic alcoholic rats .
	manualset3
225787	3	421073	7	NULL	NULL	0	NULL	ethanol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR investigation of the futile cycling of ethanol in chronic alcoholic rats .
	manualset3
225788	4	421073	7	NULL	NULL	0	NULL	 chronic alcoholic rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	NMR investigation of the futile cycling of ethanol in chronic alcoholic rats .
	manualset3
225789	1	421074	7	NULL	NULL	0	NULL	GIT1/Cat -1 ( G protein-coupled receptor kinase-interactor 1/Cool-associated , tyrosine-phosphorylated 1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Among them , GIT1/Cat -1 ( G protein-coupled receptor kinase-interactor 1/Cool-associated , tyrosine-phosphorylated 1 ) was examined further .
	manualset3
225790	1	421075	7	NULL	NULL	0	NULL	increasing evidence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence for a positive correlation between matrix metalloproteinase-2 ( MMP-2 ) activity and tumor cell invasion .
	manualset3
225791	2	421075	7	NULL	NULL	0	NULL	positive correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence for a positive correlation between matrix metalloproteinase-2 ( MMP-2 ) activity and tumor cell invasion .
	manualset3
225792	3	421075	7	NULL	NULL	0	NULL	matrix metalloproteinase-2 ( MMP-2 ) activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence for a positive correlation between matrix metalloproteinase-2 ( MMP-2 ) activity and tumor cell invasion .
	manualset3
225793	4	421075	7	NULL	NULL	0	NULL	tumor cell invasion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There is increasing evidence for a positive correlation between matrix metalloproteinase-2 ( MMP-2 ) activity and tumor cell invasion .
	manualset3
225794	1	421076	7	NULL	NULL	0	NULL	In vivo evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo evidence for increased adrenal sensitivity to adrenocorticotropin - ( 1-24 ) in the lamb fetus late in gestation .
	manualset3
225795	2	421076	7	NULL	NULL	0	NULL	increased adrenal sensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo evidence for increased adrenal sensitivity to adrenocorticotropin - ( 1-24 ) in the lamb fetus late in gestation .
	manualset3
225796	3	421076	7	NULL	NULL	0	NULL	adrenocorticotropin - ( 1-24 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo evidence for increased adrenal sensitivity to adrenocorticotropin - ( 1-24 ) in the lamb fetus late in gestation .
	manualset3
225797	4	421076	7	NULL	NULL	0	NULL	lamb fetus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo evidence for increased adrenal sensitivity to adrenocorticotropin - ( 1-24 ) in the lamb fetus late in gestation .
	manualset3
225798	5	421076	7	NULL	NULL	0	NULL	 late	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo evidence for increased adrenal sensitivity to adrenocorticotropin - ( 1-24 ) in the lamb fetus late in gestation .
	manualset3
225799	6	421076	7	NULL	NULL	0	NULL	gestation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo evidence for increased adrenal sensitivity to adrenocorticotropin - ( 1-24 ) in the lamb fetus late in gestation .
	manualset3
225903	1	421077	7	NULL	NULL	0	NULL	Nonbacterial meningitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonbacterial meningitis can not be as readily detected clinically .
	manualset3
225904	1	421078	7	NULL	NULL	0	NULL	 longer times	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	With longer times , the protein-bound carbohydrate chain becomes much more sensitive to alpha-mannosidase while remaining endo-beta-N-acetylglucosaminidase H-resistant .
	manualset3
225905	2	421078	7	NULL	NULL	0	NULL	protein-bound carbohydrate chain	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	With longer times , the protein-bound carbohydrate chain becomes much more sensitive to alpha-mannosidase while remaining endo-beta-N-acetylglucosaminidase H-resistant .
	manualset3
225906	3	421078	7	NULL	NULL	0	NULL	alpha-mannosidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	With longer times , the protein-bound carbohydrate chain becomes much more sensitive to alpha-mannosidase while remaining endo-beta-N-acetylglucosaminidase H-resistant .
	manualset3
225907	4	421078	7	NULL	NULL	NULL	NULL	endo-beta-N-acetylglucosaminidase 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	With longer times , the protein-bound carbohydrate chain becomes much more sensitive to alpha-mannosidase while remaining endo-beta-N-acetylglucosaminidase H-resistant .
	manualset3
225908	1	421079	7	NULL	NULL	0	NULL	modulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	By employing modulation on both transmission and reception , compressive sensing in ranging is extended to the direct measurement of range profiles without intermediate measurement of the return waveform .
	manualset3
225909	2	421079	7	NULL	NULL	0	NULL	transmission	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	By employing modulation on both transmission and reception , compressive sensing in ranging is extended to the direct measurement of range profiles without intermediate measurement of the return waveform .
	manualset3
225910	3	421079	7	NULL	NULL	0	NULL	reception 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	By employing modulation on both transmission and reception , compressive sensing in ranging is extended to the direct measurement of range profiles without intermediate measurement of the return waveform .
	manualset3
225911	4	421079	7	NULL	NULL	0	NULL	compressive sensing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	By employing modulation on both transmission and reception , compressive sensing in ranging is extended to the direct measurement of range profiles without intermediate measurement of the return waveform .
	manualset3
225912	5	421079	7	NULL	NULL	0	NULL	direct measurement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	By employing modulation on both transmission and reception , compressive sensing in ranging is extended to the direct measurement of range profiles without intermediate measurement of the return waveform .
	manualset3
225913	6	421079	7	NULL	NULL	0	NULL	range profiles	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	By employing modulation on both transmission and reception , compressive sensing in ranging is extended to the direct measurement of range profiles without intermediate measurement of the return waveform .
	manualset3
225914	7	421079	7	NULL	NULL	0	NULL	intermediate measurement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	By employing modulation on both transmission and reception , compressive sensing in ranging is extended to the direct measurement of range profiles without intermediate measurement of the return waveform .
	manualset3
225915	8	421079	7	NULL	NULL	0	NULL	return waveform	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	By employing modulation on both transmission and reception , compressive sensing in ranging is extended to the direct measurement of range profiles without intermediate measurement of the return waveform .
	manualset3
225916	9	421079	7	NULL	NULL	0	NULL	ranging	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	By employing modulation on both transmission and reception , compressive sensing in ranging is extended to the direct measurement of range profiles without intermediate measurement of the return waveform .
	manualset3
225917	1	421080	7	NULL	NULL	0	NULL	Bacteria 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Bacteria exhibited tropism for mucus only on explants maintained with an air interface .
	manualset3
225918	2	421080	7	NULL	NULL	0	NULL	tropism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Bacteria exhibited tropism for mucus only on explants maintained with an air interface .
	manualset3
225919	3	421080	7	NULL	NULL	0	NULL	mucus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Bacteria exhibited tropism for mucus only on explants maintained with an air interface .
	manualset3
225920	4	421080	7	NULL	NULL	NULL	NULL	 explants	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacteria exhibited tropism for mucus only on explants maintained with an air interface .
	manualset3
225922	5	421080	7	NULL	NULL	0	NULL	air interface	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Bacteria exhibited tropism for mucus only on explants maintained with an air interface .
	manualset3
225926	1	421081	7	NULL	NULL	0	NULL	PCR amplification 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To permit PCR amplification of potentially all IGHJ rearrangements , we have devised a method incorporating self-ligation of restriction endonuclease-digested DNA fragments with long-distance PCR ( long-distance , inverse PCR ( LDI-PCR ) ) .
	manualset3
225927	2	421081	7	NULL	NULL	0	NULL	IGHJ rearrangements	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To permit PCR amplification of potentially all IGHJ rearrangements , we have devised a method incorporating self-ligation of restriction endonuclease-digested DNA fragments with long-distance PCR ( long-distance , inverse PCR ( LDI-PCR ) ) .
	manualset3
225928	3	421081	7	NULL	NULL	0	NULL	method 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	To permit PCR amplification of potentially all IGHJ rearrangements , we have devised a method incorporating self-ligation of restriction endonuclease-digested DNA fragments with long-distance PCR ( long-distance , inverse PCR ( LDI-PCR ) ) .
	manualset3
225929	4	421081	7	NULL	NULL	0	NULL	self-ligation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To permit PCR amplification of potentially all IGHJ rearrangements , we have devised a method incorporating self-ligation of restriction endonuclease-digested DNA fragments with long-distance PCR ( long-distance , inverse PCR ( LDI-PCR ) ) .
	manualset3
225930	5	421081	7	NULL	NULL	0	NULL	restriction endonuclease-digested DNA fragments	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	To permit PCR amplification of potentially all IGHJ rearrangements , we have devised a method incorporating self-ligation of restriction endonuclease-digested DNA fragments with long-distance PCR ( long-distance , inverse PCR ( LDI-PCR ) ) .
	manualset3
225931	6	421081	7	NULL	NULL	0	NULL	long-distance PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To permit PCR amplification of potentially all IGHJ rearrangements , we have devised a method incorporating self-ligation of restriction endonuclease-digested DNA fragments with long-distance PCR ( long-distance , inverse PCR ( LDI-PCR ) ) .
	manualset3
225932	7	421081	7	NULL	NULL	0	NULL	long-distance	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To permit PCR amplification of potentially all IGHJ rearrangements , we have devised a method incorporating self-ligation of restriction endonuclease-digested DNA fragments with long-distance PCR ( long-distance , inverse PCR ( LDI-PCR ) ) .
	manualset3
225933	8	421081	7	NULL	NULL	0	NULL	inverse PCR ( LDI-PCR )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	To permit PCR amplification of potentially all IGHJ rearrangements , we have devised a method incorporating self-ligation of restriction endonuclease-digested DNA fragments with long-distance PCR ( long-distance , inverse PCR ( LDI-PCR ) ) .
	manualset3
225944	1	421082	7	NULL	NULL	0	NULL	 deformities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The commonest deformities and disabilities of the thumb seen in this country are secondary to ulnar and median nerve paralysis because of leprosy .
	manualset3
225945	2	421082	7	NULL	NULL	0	NULL	disabilities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The commonest deformities and disabilities of the thumb seen in this country are secondary to ulnar and median nerve paralysis because of leprosy .
	manualset3
225946	3	421082	7	NULL	NULL	0	NULL	thumb	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The commonest deformities and disabilities of the thumb seen in this country are secondary to ulnar and median nerve paralysis because of leprosy .
	manualset3
225947	4	421082	7	NULL	NULL	0	NULL	country	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The commonest deformities and disabilities of the thumb seen in this country are secondary to ulnar and median nerve paralysis because of leprosy .
	manualset3
225948	5	421082	7	NULL	NULL	NULL	NULL	ulnar nerve paralysis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The commonest deformities and disabilities of the thumb seen in this country are secondary to ulnar and median nerve paralysis because of leprosy .
	manualset3
225951	6	421082	7	NULL	NULL	NULL	NULL	median nerve paralysis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The commonest deformities and disabilities of the thumb seen in this country are secondary to ulnar and median nerve paralysis because of leprosy .
	manualset3
225954	7	421082	7	NULL	NULL	0	NULL	leprosy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The commonest deformities and disabilities of the thumb seen in this country are secondary to ulnar and median nerve paralysis because of leprosy .
	manualset3
225958	1	421083	7	NULL	NULL	0	NULL	Nasal cavities 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Nasal cavities of rats exposed to 25 or 76 ppm revealed evidence of inflammatory cell infiltration , focal hyperplasia , and squamous metaplasia in the respiratory epithelium of the anterior nasal turbinates .
	manualset3
225959	2	421083	7	NULL	NULL	0	NULL	 rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Nasal cavities of rats exposed to 25 or 76 ppm revealed evidence of inflammatory cell infiltration , focal hyperplasia , and squamous metaplasia in the respiratory epithelium of the anterior nasal turbinates .
	manualset3
225960	3	421083	7	NULL	NULL	0	NULL	25 ppm	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nasal cavities of rats exposed to 25 or 76 ppm revealed evidence of inflammatory cell infiltration , focal hyperplasia , and squamous metaplasia in the respiratory epithelium of the anterior nasal turbinates .
	manualset3
225961	4	421083	7	NULL	NULL	0	NULL	76 ppm	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nasal cavities of rats exposed to 25 or 76 ppm revealed evidence of inflammatory cell infiltration , focal hyperplasia , and squamous metaplasia in the respiratory epithelium of the anterior nasal turbinates .
	manualset3
225962	5	421083	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nasal cavities of rats exposed to 25 or 76 ppm revealed evidence of inflammatory cell infiltration , focal hyperplasia , and squamous metaplasia in the respiratory epithelium of the anterior nasal turbinates .
	manualset3
225964	6	421083	7	NULL	NULL	0	NULL	inflammatory cell infiltration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nasal cavities of rats exposed to 25 or 76 ppm revealed evidence of inflammatory cell infiltration , focal hyperplasia , and squamous metaplasia in the respiratory epithelium of the anterior nasal turbinates .
	manualset3
225966	7	421083	7	NULL	NULL	0	NULL	focal hyperplasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nasal cavities of rats exposed to 25 or 76 ppm revealed evidence of inflammatory cell infiltration , focal hyperplasia , and squamous metaplasia in the respiratory epithelium of the anterior nasal turbinates .
	manualset3
225967	8	421083	7	NULL	NULL	0	NULL	squamous metaplasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nasal cavities of rats exposed to 25 or 76 ppm revealed evidence of inflammatory cell infiltration , focal hyperplasia , and squamous metaplasia in the respiratory epithelium of the anterior nasal turbinates .
	manualset3
225968	9	421083	7	NULL	NULL	0	NULL	respiratory epithelium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Nasal cavities of rats exposed to 25 or 76 ppm revealed evidence of inflammatory cell infiltration , focal hyperplasia , and squamous metaplasia in the respiratory epithelium of the anterior nasal turbinates .
	manualset3
225972	10	421083	7	NULL	NULL	0	NULL	anterior nasal turbinates	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Nasal cavities of rats exposed to 25 or 76 ppm revealed evidence of inflammatory cell infiltration , focal hyperplasia , and squamous metaplasia in the respiratory epithelium of the anterior nasal turbinates .
	manualset3
225982	1	421084	7	NULL	NULL	0	NULL	Idesolide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Idesolide significantly reduced nitric oxide production induced by lipopolysaccharide in BV2 microglial cells .
	manualset3
225983	2	421084	7	NULL	NULL	0	NULL	nitric oxide production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Idesolide significantly reduced nitric oxide production induced by lipopolysaccharide in BV2 microglial cells .
	manualset3
225984	3	421084	7	NULL	NULL	0	NULL	 lipopolysaccharide	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Idesolide significantly reduced nitric oxide production induced by lipopolysaccharide in BV2 microglial cells .
	manualset3
225985	4	421084	7	NULL	NULL	0	NULL	BV2 microglial cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Idesolide significantly reduced nitric oxide production induced by lipopolysaccharide in BV2 microglial cells .
	manualset3
225986	1	421085	7	NULL	NULL	0	NULL	 planning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For the planning of mediation processes it is mandatory that the mediator knows the basics of mediation ( progressing steps , methods , techniques ) and is also aware of the psychological and legal backgrounds .
	manualset3
225987	2	421085	7	NULL	NULL	0	NULL	mediation processes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For the planning of mediation processes it is mandatory that the mediator knows the basics of mediation ( progressing steps , methods , techniques ) and is also aware of the psychological and legal backgrounds .
	manualset3
225988	3	421085	7	NULL	NULL	0	NULL	mediator	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	For the planning of mediation processes it is mandatory that the mediator knows the basics of mediation ( progressing steps , methods , techniques ) and is also aware of the psychological and legal backgrounds .
	manualset3
225989	4	421085	7	NULL	NULL	0	NULL	 basics	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For the planning of mediation processes it is mandatory that the mediator knows the basics of mediation ( progressing steps , methods , techniques ) and is also aware of the psychological and legal backgrounds .
	manualset3
225990	5	421085	7	NULL	NULL	0	NULL	 mediation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For the planning of mediation processes it is mandatory that the mediator knows the basics of mediation ( progressing steps , methods , techniques ) and is also aware of the psychological and legal backgrounds .
	manualset3
225991	6	421085	7	NULL	NULL	0	NULL	progressing steps	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For the planning of mediation processes it is mandatory that the mediator knows the basics of mediation ( progressing steps , methods , techniques ) and is also aware of the psychological and legal backgrounds .
	manualset3
225992	7	421085	7	NULL	NULL	0	NULL	methods	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	For the planning of mediation processes it is mandatory that the mediator knows the basics of mediation ( progressing steps , methods , techniques ) and is also aware of the psychological and legal backgrounds .
	manualset3
225993	8	421085	7	NULL	NULL	0	NULL	techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the planning of mediation processes it is mandatory that the mediator knows the basics of mediation ( progressing steps , methods , techniques ) and is also aware of the psychological and legal backgrounds .
	manualset3
225994	9	421085	7	NULL	NULL	0	NULL	psychological background	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For the planning of mediation processes it is mandatory that the mediator knows the basics of mediation ( progressing steps , methods , techniques ) and is also aware of the psychological and legal backgrounds .
	manualset3
225995	10	421085	7	NULL	NULL	0	NULL	legal backgrounds	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For the planning of mediation processes it is mandatory that the mediator knows the basics of mediation ( progressing steps , methods , techniques ) and is also aware of the psychological and legal backgrounds .
	manualset3
226042	1	421086	7	NULL	NULL	0	NULL	cranial region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cranial region , the great majority ( 52 to 63 % ) of myofibres were type IIA .
	manualset3
226043	2	421086	7	NULL	NULL	0	NULL	great majority 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cranial region , the great majority ( 52 to 63 % ) of myofibres were type IIA .
	manualset3
226044	3	421086	7	NULL	NULL	0	NULL	 52 to 63 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cranial region , the great majority ( 52 to 63 % ) of myofibres were type IIA .
	manualset3
226045	4	421086	7	NULL	NULL	0	NULL	myofibres	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cranial region , the great majority ( 52 to 63 % ) of myofibres were type IIA .
	manualset3
226046	5	421086	7	NULL	NULL	0	NULL	IIA	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In the cranial region , the great majority ( 52 to 63 % ) of myofibres were type IIA .
	manualset3
226047	1	421087	7	NULL	NULL	0	NULL	 role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of FDG PET in management of neck metastasis from head-and-neck cancer after definitive radiation treatment .
	manualset3
226048	2	421087	7	NULL	NULL	0	NULL	FDG PET	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of FDG PET in management of neck metastasis from head-and-neck cancer after definitive radiation treatment .
	manualset3
226049	3	421087	7	NULL	NULL	0	NULL	management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of FDG PET in management of neck metastasis from head-and-neck cancer after definitive radiation treatment .
	manualset3
226050	4	421087	7	NULL	NULL	0	NULL	neck metastasis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of FDG PET in management of neck metastasis from head-and-neck cancer after definitive radiation treatment .
	manualset3
226051	5	421087	7	NULL	NULL	0	NULL	head-and-neck cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of FDG PET in management of neck metastasis from head-and-neck cancer after definitive radiation treatment .
	manualset3
226052	6	421087	7	NULL	NULL	0	NULL	radiation treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of FDG PET in management of neck metastasis from head-and-neck cancer after definitive radiation treatment .
	manualset3
226053	1	421088	7	NULL	NULL	0	NULL	 substances	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These substances showed strong anti-HSV-1 activity in vitro but only 3 inhibited the reverse transcriptase enzyme of HIV-1 .
	manualset3
226054	2	421088	7	NULL	NULL	0	NULL	strong anti-HSV-1 activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These substances showed strong anti-HSV-1 activity in vitro but only 3 inhibited the reverse transcriptase enzyme of HIV-1 .
	manualset3
226055	3	421088	7	NULL	NULL	0	NULL	 3 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These substances showed strong anti-HSV-1 activity in vitro but only 3 inhibited the reverse transcriptase enzyme of HIV-1 .
	manualset3
226056	4	421088	7	NULL	NULL	0	NULL	 reverse transcriptase enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These substances showed strong anti-HSV-1 activity in vitro but only 3 inhibited the reverse transcriptase enzyme of HIV-1 .
	manualset3
226057	5	421088	7	NULL	NULL	0	NULL	HIV-1	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These substances showed strong anti-HSV-1 activity in vitro but only 3 inhibited the reverse transcriptase enzyme of HIV-1 .
	manualset3
226058	1	421089	7	NULL	NULL	0	NULL	one 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among them , the one most frequently implicated in stomach cancer is the abnormal expression and amplification of the c-met gene .
	manualset3
226059	2	421089	7	NULL	NULL	0	NULL	stomach cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Among them , the one most frequently implicated in stomach cancer is the abnormal expression and amplification of the c-met gene .
	manualset3
226060	3	421089	7	NULL	NULL	0	NULL	abnormal expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among them , the one most frequently implicated in stomach cancer is the abnormal expression and amplification of the c-met gene .
	manualset3
226061	4	421089	7	NULL	NULL	0	NULL	amplification	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among them , the one most frequently implicated in stomach cancer is the abnormal expression and amplification of the c-met gene .
	manualset3
226062	5	421089	7	NULL	NULL	0	NULL	c-met gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Among them , the one most frequently implicated in stomach cancer is the abnormal expression and amplification of the c-met gene .
	manualset3
226063	1	421090	7	NULL	NULL	0	NULL	 use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	By use of ( 7235 x TM-1 ) F2 in Nanjing and College Station , USA , and ( 7235 x TM-1 ) F3 in Nanjing and Hainan .
	manualset3
226064	2	421090	7	NULL	NULL	0	NULL	( 7235 x TM-1 ) F2 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	By use of ( 7235 x TM-1 ) F2 in Nanjing and College Station , USA , and ( 7235 x TM-1 ) F3 in Nanjing and Hainan .
	manualset3
226065	3	421090	7	NULL	NULL	0	NULL	Nanjing 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	By use of ( 7235 x TM-1 ) F2 in Nanjing and College Station , USA , and ( 7235 x TM-1 ) F3 in Nanjing and Hainan .
	manualset3
226066	4	421090	7	NULL	NULL	0	NULL	College Station	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	By use of ( 7235 x TM-1 ) F2 in Nanjing and College Station , USA , and ( 7235 x TM-1 ) F3 in Nanjing and Hainan .
	manualset3
226067	5	421090	7	NULL	NULL	0	NULL	USA	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	By use of ( 7235 x TM-1 ) F2 in Nanjing and College Station , USA , and ( 7235 x TM-1 ) F3 in Nanjing and Hainan .
	manualset3
226068	6	421090	7	NULL	NULL	0	NULL	( 7235 x TM-1 ) F3	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	By use of ( 7235 x TM-1 ) F2 in Nanjing and College Station , USA , and ( 7235 x TM-1 ) F3 in Nanjing and Hainan .
	manualset3
226069	7	421090	7	NULL	NULL	0	NULL	Nanjing	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	By use of ( 7235 x TM-1 ) F2 in Nanjing and College Station , USA , and ( 7235 x TM-1 ) F3 in Nanjing and Hainan .
	manualset3
226070	8	421090	7	NULL	NULL	0	NULL	Hainan	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	By use of ( 7235 x TM-1 ) F2 in Nanjing and College Station , USA , and ( 7235 x TM-1 ) F3 in Nanjing and Hainan .
	manualset3
226071	1	421091	7	NULL	NULL	0	NULL	Captopril ( SQ 14225 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Captopril ( SQ 14225 ) is an inhibitor of angiotensin I-converting enzyme ( ACE ) .
	manualset3
226072	2	421091	7	NULL	NULL	0	NULL	inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Captopril ( SQ 14225 ) is an inhibitor of angiotensin I-converting enzyme ( ACE ) .
	manualset3
226073	3	421091	7	NULL	NULL	0	NULL	angiotensin I-converting enzyme ( ACE )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Captopril ( SQ 14225 ) is an inhibitor of angiotensin I-converting enzyme ( ACE ) .
	manualset3
226074	1	421092	7	NULL	NULL	0	NULL	Recent therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Recent therapy of leukemia in childhood ) .
	manualset3
226075	2	421092	7	NULL	NULL	0	NULL	leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Recent therapy of leukemia in childhood ) .
	manualset3
226076	3	421092	7	NULL	NULL	0	NULL	 childhood	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	( Recent therapy of leukemia in childhood ) .
	manualset3
226077	1	421093	7	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation between RHF and the sum of TBARS and GPXA was also highly significant in both kidney and liver homogenates .
	manualset3
226078	2	421093	7	NULL	NULL	0	NULL	RHF	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation between RHF and the sum of TBARS and GPXA was also highly significant in both kidney and liver homogenates .
	manualset3
226079	3	421093	7	NULL	NULL	0	NULL	sum	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation between RHF and the sum of TBARS and GPXA was also highly significant in both kidney and liver homogenates .
	manualset3
226080	4	421093	7	NULL	NULL	0	NULL	TBARS 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation between RHF and the sum of TBARS and GPXA was also highly significant in both kidney and liver homogenates .
	manualset3
226081	5	421093	7	NULL	NULL	0	NULL	GPXA	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation between RHF and the sum of TBARS and GPXA was also highly significant in both kidney and liver homogenates .
	manualset3
226082	6	421093	7	NULL	NULL	0	NULL	kidney	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation between RHF and the sum of TBARS and GPXA was also highly significant in both kidney and liver homogenates .
	manualset3
226083	7	421093	7	NULL	NULL	0	NULL	liver homogenates	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	The correlation between RHF and the sum of TBARS and GPXA was also highly significant in both kidney and liver homogenates .
	manualset3
226084	1	421094	7	NULL	NULL	NULL	NULL	Iron/dextran sulfate multilayered microcapsules	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Iron/dextran sulfate multilayered microcapsules for controlled release of 10-hydroxycamptothecin .
	manualset3
226085	2	421094	7	NULL	NULL	0	NULL	controlled release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Iron/dextran sulfate multilayered microcapsules for controlled release of 10-hydroxycamptothecin .
	manualset3
226086	3	421094	7	NULL	NULL	0	NULL	10-hydroxycamptothecin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Iron/dextran sulfate multilayered microcapsules for controlled release of 10-hydroxycamptothecin .
	manualset3
226087	1	421095	7	NULL	NULL	0	NULL	growth increase	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This growth increase was suppressed by MIF inhibition .
	manualset3
226088	2	421095	7	NULL	NULL	0	NULL	MIF inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This growth increase was suppressed by MIF inhibition .
	manualset3
226089	1	421096	7	NULL	NULL	0	NULL	Direct association	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct association of presenilin-1 with beta-catenin .
	manualset3
226090	2	421096	7	NULL	NULL	0	NULL	presenilin-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct association of presenilin-1 with beta-catenin .
	manualset3
226091	3	421096	7	NULL	NULL	0	NULL	beta-catenin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct association of presenilin-1 with beta-catenin .
	manualset3
226092	1	421097	7	NULL	NULL	0	NULL	normal cholangiocyte line	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A normal cholangiocyte line showed the induction of AID transcripts after stimulation with TNF-alpha , whereas ganp transcripts appeared constitutively in this cell line .
	manualset3
226093	2	421097	7	NULL	NULL	0	NULL	induction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A normal cholangiocyte line showed the induction of AID transcripts after stimulation with TNF-alpha , whereas ganp transcripts appeared constitutively in this cell line .
	manualset3
226094	3	421097	7	NULL	NULL	0	NULL	AID transcripts	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A normal cholangiocyte line showed the induction of AID transcripts after stimulation with TNF-alpha , whereas ganp transcripts appeared constitutively in this cell line .
	manualset3
226095	4	421097	7	NULL	NULL	0	NULL	stimulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A normal cholangiocyte line showed the induction of AID transcripts after stimulation with TNF-alpha , whereas ganp transcripts appeared constitutively in this cell line .
	manualset3
226096	5	421097	7	NULL	NULL	0	NULL	 TNF-alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A normal cholangiocyte line showed the induction of AID transcripts after stimulation with TNF-alpha , whereas ganp transcripts appeared constitutively in this cell line .
	manualset3
226097	6	421097	7	NULL	NULL	0	NULL	ganp transcripts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A normal cholangiocyte line showed the induction of AID transcripts after stimulation with TNF-alpha , whereas ganp transcripts appeared constitutively in this cell line .
	manualset3
226098	7	421097	7	NULL	NULL	0	NULL	cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A normal cholangiocyte line showed the induction of AID transcripts after stimulation with TNF-alpha , whereas ganp transcripts appeared constitutively in this cell line .
	manualset3
226099	1	421098	7	NULL	NULL	0	NULL	one 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these , one very pleiotropic syndrome results from deficiencies in an array of cytokine signaling pathways utilizing a cytokine receptor common gamma chain , gammac , and the tyrosine kinase Jak3 .
	manualset3
226100	2	421098	7	NULL	NULL	0	NULL	pleiotropic syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these , one very pleiotropic syndrome results from deficiencies in an array of cytokine signaling pathways utilizing a cytokine receptor common gamma chain , gammac , and the tyrosine kinase Jak3 .
	manualset3
226101	3	421098	7	NULL	NULL	0	NULL	deficiencies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these , one very pleiotropic syndrome results from deficiencies in an array of cytokine signaling pathways utilizing a cytokine receptor common gamma chain , gammac , and the tyrosine kinase Jak3 .
	manualset3
226102	4	421098	7	NULL	NULL	0	NULL	array	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these , one very pleiotropic syndrome results from deficiencies in an array of cytokine signaling pathways utilizing a cytokine receptor common gamma chain , gammac , and the tyrosine kinase Jak3 .
	manualset3
226103	5	421098	7	NULL	NULL	0	NULL	cytokine signaling pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these , one very pleiotropic syndrome results from deficiencies in an array of cytokine signaling pathways utilizing a cytokine receptor common gamma chain , gammac , and the tyrosine kinase Jak3 .
	manualset3
226104	6	421098	7	NULL	NULL	0	NULL	cytokine receptor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these , one very pleiotropic syndrome results from deficiencies in an array of cytokine signaling pathways utilizing a cytokine receptor common gamma chain , gammac , and the tyrosine kinase Jak3 .
	manualset3
226105	7	421098	7	NULL	NULL	0	NULL	gamma chain , gammac	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these , one very pleiotropic syndrome results from deficiencies in an array of cytokine signaling pathways utilizing a cytokine receptor common gamma chain , gammac , and the tyrosine kinase Jak3 .
	manualset3
226106	8	421098	7	NULL	NULL	0	NULL	tyrosine kinase Jak3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these , one very pleiotropic syndrome results from deficiencies in an array of cytokine signaling pathways utilizing a cytokine receptor common gamma chain , gammac , and the tyrosine kinase Jak3 .
	manualset3
226107	1	421099	7	NULL	NULL	0	NULL	Health services	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Health services for undocumented migrants highlight the complex politics of the `` right to health '' .
	manualset3
226108	2	421099	7	NULL	NULL	0	NULL	undocumented migrants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Health services for undocumented migrants highlight the complex politics of the `` right to health '' .
	manualset3
226109	3	421099	7	NULL	NULL	0	NULL	complex politics 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Health services for undocumented migrants highlight the complex politics of the `` right to health '' .
	manualset3
226110	4	421099	7	NULL	NULL	0	NULL	`` right to health ''	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Health services for undocumented migrants highlight the complex politics of the `` right to health '' .
	manualset3
226111	1	421100	7	NULL	NULL	0	NULL	 3 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	For 3 months to 3 years , 22 subjects were examined , another patient had a relapse 3 months following surgery .
	manualset3
226112	2	421100	7	NULL	NULL	0	NULL	3 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	For 3 months to 3 years , 22 subjects were examined , another patient had a relapse 3 months following surgery .
	manualset3
226113	3	421100	7	NULL	NULL	0	NULL	22 subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	For 3 months to 3 years , 22 subjects were examined , another patient had a relapse 3 months following surgery .
	manualset3
226114	4	421100	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	For 3 months to 3 years , 22 subjects were examined , another patient had a relapse 3 months following surgery .
	manualset3
226115	5	421100	7	NULL	NULL	0	NULL	relapse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For 3 months to 3 years , 22 subjects were examined , another patient had a relapse 3 months following surgery .
	manualset3
226116	6	421100	7	NULL	NULL	0	NULL	3 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	For 3 months to 3 years , 22 subjects were examined , another patient had a relapse 3 months following surgery .
	manualset3
226117	7	421100	7	NULL	NULL	0	NULL	surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For 3 months to 3 years , 22 subjects were examined , another patient had a relapse 3 months following surgery .
	manualset3
226118	1	421101	7	NULL	NULL	0	NULL	Three patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Three patients , one of whom has been previously reported , had erythematous papules and nodules of the face and upper part of the chest during cyclosporine therapy for inflammatory skin diseases .
	manualset3
226119	2	421101	7	NULL	NULL	0	NULL	 one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Three patients , one of whom has been previously reported , had erythematous papules and nodules of the face and upper part of the chest during cyclosporine therapy for inflammatory skin diseases .
	manualset3
226120	3	421101	7	NULL	NULL	0	NULL	erythematous papules 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Three patients , one of whom has been previously reported , had erythematous papules and nodules of the face and upper part of the chest during cyclosporine therapy for inflammatory skin diseases .
	manualset3
226121	4	421101	7	NULL	NULL	0	NULL	nodules of the face	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Three patients , one of whom has been previously reported , had erythematous papules and nodules of the face and upper part of the chest during cyclosporine therapy for inflammatory skin diseases .
	manualset3
226122	5	421101	7	NULL	NULL	0	NULL	upper part of the chest	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Three patients , one of whom has been previously reported , had erythematous papules and nodules of the face and upper part of the chest during cyclosporine therapy for inflammatory skin diseases .
	manualset3
226123	6	421101	7	NULL	NULL	0	NULL	cyclosporine therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Three patients , one of whom has been previously reported , had erythematous papules and nodules of the face and upper part of the chest during cyclosporine therapy for inflammatory skin diseases .
	manualset3
226124	7	421101	7	NULL	NULL	0	NULL	inflammatory skin diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Three patients , one of whom has been previously reported , had erythematous papules and nodules of the face and upper part of the chest during cyclosporine therapy for inflammatory skin diseases .
	manualset3
226125	1	421102	7	NULL	NULL	0	NULL	Aging	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Aging , source , and decision criteria : when false fame errors do and do not occur .
	manualset3
226126	2	421102	7	NULL	NULL	0	NULL	 source	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Aging , source , and decision criteria : when false fame errors do and do not occur .
	manualset3
226127	3	421102	7	NULL	NULL	0	NULL	decision criteria	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Aging , source , and decision criteria : when false fame errors do and do not occur .
	manualset3
226128	4	421102	7	NULL	NULL	0	NULL	false fame errors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Aging , source , and decision criteria : when false fame errors do and do not occur .
	manualset3
226184	1	421103	7	NULL	NULL	0	NULL	Targeting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Targeting tumors with LIGHT to generate metastasis-clearing immunity .
	manualset3
226185	2	421103	7	NULL	NULL	0	NULL	tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Targeting tumors with LIGHT to generate metastasis-clearing immunity .
	manualset3
226186	3	421103	7	NULL	NULL	0	NULL	LIGHT 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Targeting tumors with LIGHT to generate metastasis-clearing immunity .
	manualset3
226187	4	421103	7	NULL	NULL	0	NULL	metastasis-clearing immunity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Targeting tumors with LIGHT to generate metastasis-clearing immunity .
	manualset3
226188	1	421104	7	NULL	NULL	0	NULL	GPCR targets	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these GPCR targets are the receptors for peptides like bradykinin , chemokines , complement anaphylatoxins , corticotropin releasing factor , endothelins , melanocortins , tachykinins , urocortins , as well as the protease activated receptors ( PARs ) .
	manualset3
226189	2	421104	7	NULL	NULL	0	NULL	 receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these GPCR targets are the receptors for peptides like bradykinin , chemokines , complement anaphylatoxins , corticotropin releasing factor , endothelins , melanocortins , tachykinins , urocortins , as well as the protease activated receptors ( PARs ) .
	manualset3
226190	3	421104	7	NULL	NULL	0	NULL	peptides 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these GPCR targets are the receptors for peptides like bradykinin , chemokines , complement anaphylatoxins , corticotropin releasing factor , endothelins , melanocortins , tachykinins , urocortins , as well as the protease activated receptors ( PARs ) .
	manualset3
226191	4	421104	7	NULL	NULL	0	NULL	bradykinin	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these GPCR targets are the receptors for peptides like bradykinin , chemokines , complement anaphylatoxins , corticotropin releasing factor , endothelins , melanocortins , tachykinins , urocortins , as well as the protease activated receptors ( PARs ) .
	manualset3
226192	5	421104	7	NULL	NULL	0	NULL	chemokines	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these GPCR targets are the receptors for peptides like bradykinin , chemokines , complement anaphylatoxins , corticotropin releasing factor , endothelins , melanocortins , tachykinins , urocortins , as well as the protease activated receptors ( PARs ) .
	manualset3
226193	6	421104	7	NULL	NULL	0	NULL	complement anaphylatoxins	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these GPCR targets are the receptors for peptides like bradykinin , chemokines , complement anaphylatoxins , corticotropin releasing factor , endothelins , melanocortins , tachykinins , urocortins , as well as the protease activated receptors ( PARs ) .
	manualset3
226194	7	421104	7	NULL	NULL	0	NULL	corticotropin releasing factor	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these GPCR targets are the receptors for peptides like bradykinin , chemokines , complement anaphylatoxins , corticotropin releasing factor , endothelins , melanocortins , tachykinins , urocortins , as well as the protease activated receptors ( PARs ) .
	manualset3
226195	8	421104	7	NULL	NULL	0	NULL	 endothelins	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these GPCR targets are the receptors for peptides like bradykinin , chemokines , complement anaphylatoxins , corticotropin releasing factor , endothelins , melanocortins , tachykinins , urocortins , as well as the protease activated receptors ( PARs ) .
	manualset3
226196	9	421104	7	NULL	NULL	0	NULL	melanocortins	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these GPCR targets are the receptors for peptides like bradykinin , chemokines , complement anaphylatoxins , corticotropin releasing factor , endothelins , melanocortins , tachykinins , urocortins , as well as the protease activated receptors ( PARs ) .
	manualset3
226197	10	421104	7	NULL	NULL	0	NULL	 tachykinins 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these GPCR targets are the receptors for peptides like bradykinin , chemokines , complement anaphylatoxins , corticotropin releasing factor , endothelins , melanocortins , tachykinins , urocortins , as well as the protease activated receptors ( PARs ) .
	manualset3
226198	11	421104	7	NULL	NULL	0	NULL	urocortins	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these GPCR targets are the receptors for peptides like bradykinin , chemokines , complement anaphylatoxins , corticotropin releasing factor , endothelins , melanocortins , tachykinins , urocortins , as well as the protease activated receptors ( PARs ) .
	manualset3
226199	12	421104	7	NULL	NULL	0	NULL	protease activated receptors ( PARs )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these GPCR targets are the receptors for peptides like bradykinin , chemokines , complement anaphylatoxins , corticotropin releasing factor , endothelins , melanocortins , tachykinins , urocortins , as well as the protease activated receptors ( PARs ) .
	manualset3
226200	1	421105	7	NULL	NULL	0	NULL	 elevated serum levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that elevated serum levels of sVCAM-1 might serve as a possible marker for detecting pre-clinical or early cancer .
	manualset3
226201	2	421105	7	NULL	NULL	0	NULL	sVCAM-1	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that elevated serum levels of sVCAM-1 might serve as a possible marker for detecting pre-clinical or early cancer .
	manualset3
226202	3	421105	7	NULL	NULL	0	NULL	possible marker 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that elevated serum levels of sVCAM-1 might serve as a possible marker for detecting pre-clinical or early cancer .
	manualset3
226203	4	421105	7	NULL	NULL	0	NULL	pre-clinical cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that elevated serum levels of sVCAM-1 might serve as a possible marker for detecting pre-clinical or early cancer .
	manualset3
226204	5	421105	7	NULL	NULL	0	NULL	early cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that elevated serum levels of sVCAM-1 might serve as a possible marker for detecting pre-clinical or early cancer .
	manualset3
226205	1	421106	7	NULL	NULL	0	NULL	perforant pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The perforant pathway originates from cells in the entorhinal cortex and relays sensory information from the neocortex to the hippocampus , a region critical for memory function .
	manualset3
226206	2	421106	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The perforant pathway originates from cells in the entorhinal cortex and relays sensory information from the neocortex to the hippocampus , a region critical for memory function .
	manualset3
226207	3	421106	7	NULL	NULL	0	NULL	entorhinal cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The perforant pathway originates from cells in the entorhinal cortex and relays sensory information from the neocortex to the hippocampus , a region critical for memory function .
	manualset3
226208	4	421106	7	NULL	NULL	0	NULL	sensory information	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The perforant pathway originates from cells in the entorhinal cortex and relays sensory information from the neocortex to the hippocampus , a region critical for memory function .
	manualset3
226209	5	421106	7	NULL	NULL	0	NULL	neocortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The perforant pathway originates from cells in the entorhinal cortex and relays sensory information from the neocortex to the hippocampus , a region critical for memory function .
	manualset3
226210	6	421106	7	NULL	NULL	0	NULL	hippocampus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The perforant pathway originates from cells in the entorhinal cortex and relays sensory information from the neocortex to the hippocampus , a region critical for memory function .
	manualset3
226211	7	421106	7	NULL	NULL	0	NULL	region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The perforant pathway originates from cells in the entorhinal cortex and relays sensory information from the neocortex to the hippocampus , a region critical for memory function .
	manualset3
226212	8	421106	7	NULL	NULL	0	NULL	memory function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The perforant pathway originates from cells in the entorhinal cortex and relays sensory information from the neocortex to the hippocampus , a region critical for memory function .
	manualset3
226213	1	421107	7	NULL	NULL	0	NULL	Osteopathic theory	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Osteopathic theory : a strategy for curriculum integration .
	manualset3
226214	2	421107	7	NULL	NULL	0	NULL	strategy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Osteopathic theory : a strategy for curriculum integration .
	manualset3
226215	3	421107	7	NULL	NULL	0	NULL	curriculum integration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Osteopathic theory : a strategy for curriculum integration .
	manualset3
226216	1	421108	7	NULL	NULL	0	NULL	penetration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The penetration and distribution in various areas of cat brain of 14C-DL-DOPA and/or its derivatives was studied by the autoradiographic technique .
	manualset3
226217	2	421108	7	NULL	NULL	0	NULL	distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The penetration and distribution in various areas of cat brain of 14C-DL-DOPA and/or its derivatives was studied by the autoradiographic technique .
	manualset3
226218	3	421108	7	NULL	NULL	0	NULL	various areas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The penetration and distribution in various areas of cat brain of 14C-DL-DOPA and/or its derivatives was studied by the autoradiographic technique .
	manualset3
226219	4	421108	7	NULL	NULL	0	NULL	cat brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The penetration and distribution in various areas of cat brain of 14C-DL-DOPA and/or its derivatives was studied by the autoradiographic technique .
	manualset3
226220	5	421108	7	NULL	NULL	0	NULL	14C-DL-DOPA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The penetration and distribution in various areas of cat brain of 14C-DL-DOPA and/or its derivatives was studied by the autoradiographic technique .
	manualset3
226221	6	421108	7	NULL	NULL	0	NULL	derivatives	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The penetration and distribution in various areas of cat brain of 14C-DL-DOPA and/or its derivatives was studied by the autoradiographic technique .
	manualset3
226222	7	421108	7	NULL	NULL	0	NULL	autoradiographic technique 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The penetration and distribution in various areas of cat brain of 14C-DL-DOPA and/or its derivatives was studied by the autoradiographic technique .
	manualset3
226223	1	421109	7	NULL	NULL	0	NULL	Turkey	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In Turkey , 167 , 000 individuals are believed to be victims of animal bites annually .
	manualset3
226224	2	421109	7	NULL	NULL	0	NULL	167 , 000 individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In Turkey , 167 , 000 individuals are believed to be victims of animal bites annually .
	manualset3
226225	3	421109	7	NULL	NULL	0	NULL	victims	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In Turkey , 167 , 000 individuals are believed to be victims of animal bites annually .
	manualset3
226226	4	421109	7	NULL	NULL	0	NULL	animal bites 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In Turkey , 167 , 000 individuals are believed to be victims of animal bites annually .
	manualset3
226227	1	421110	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are similar to those obtained for the inactive S. L. E. ( 9 ) .
	manualset3
226228	2	421110	7	NULL	NULL	0	NULL	 inactive S. L. E. 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are similar to those obtained for the inactive S. L. E. ( 9 ) .
	manualset3
226229	3	421110	7	NULL	NULL	0	NULL	similar	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	These results are similar to those obtained for the inactive S. L. E. ( 9 ) .
	manualset3
226230	1	421111	7	NULL	NULL	0	NULL	conjunction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether used alone or in conjunction with surgery and ( or ) external irradiation , brachytherapy has contributed to the development of organ conserving treatment for cancer , notably and more recently , for carcinoma of the breast , bladder and buccal cavity , in addition to its traditional applications in gynecological and cutaneous cancers .
	manualset3
226231	2	421111	7	NULL	NULL	NULL	NULL	 surgery	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Whether used alone or in conjunction with surgery and ( or ) external irradiation , brachytherapy has contributed to the development of organ conserving treatment for cancer , notably and more recently , for carcinoma of the breast , bladder and buccal cavity , in addition to its traditional applications in gynecological and cutaneous cancers .
	manualset3
226232	3	421111	7	NULL	NULL	0	NULL	external irradiation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether used alone or in conjunction with surgery and ( or ) external irradiation , brachytherapy has contributed to the development of organ conserving treatment for cancer , notably and more recently , for carcinoma of the breast , bladder and buccal cavity , in addition to its traditional applications in gynecological and cutaneous cancers .
	manualset3
226233	4	421111	7	NULL	NULL	0	NULL	brachytherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether used alone or in conjunction with surgery and ( or ) external irradiation , brachytherapy has contributed to the development of organ conserving treatment for cancer , notably and more recently , for carcinoma of the breast , bladder and buccal cavity , in addition to its traditional applications in gynecological and cutaneous cancers .
	manualset3
226234	5	421111	7	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether used alone or in conjunction with surgery and ( or ) external irradiation , brachytherapy has contributed to the development of organ conserving treatment for cancer , notably and more recently , for carcinoma of the breast , bladder and buccal cavity , in addition to its traditional applications in gynecological and cutaneous cancers .
	manualset3
226235	6	421111	7	NULL	NULL	0	NULL	organ	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether used alone or in conjunction with surgery and ( or ) external irradiation , brachytherapy has contributed to the development of organ conserving treatment for cancer , notably and more recently , for carcinoma of the breast , bladder and buccal cavity , in addition to its traditional applications in gynecological and cutaneous cancers .
	manualset3
226236	7	421111	7	NULL	NULL	0	NULL	 treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether used alone or in conjunction with surgery and ( or ) external irradiation , brachytherapy has contributed to the development of organ conserving treatment for cancer , notably and more recently , for carcinoma of the breast , bladder and buccal cavity , in addition to its traditional applications in gynecological and cutaneous cancers .
	manualset3
226237	8	421111	7	NULL	NULL	0	NULL	cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether used alone or in conjunction with surgery and ( or ) external irradiation , brachytherapy has contributed to the development of organ conserving treatment for cancer , notably and more recently , for carcinoma of the breast , bladder and buccal cavity , in addition to its traditional applications in gynecological and cutaneous cancers .
	manualset3
226238	9	421111	7	NULL	NULL	0	NULL	carcinoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether used alone or in conjunction with surgery and ( or ) external irradiation , brachytherapy has contributed to the development of organ conserving treatment for cancer , notably and more recently , for carcinoma of the breast , bladder and buccal cavity , in addition to its traditional applications in gynecological and cutaneous cancers .
	manualset3
226239	10	421111	7	NULL	NULL	0	NULL	breast 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether used alone or in conjunction with surgery and ( or ) external irradiation , brachytherapy has contributed to the development of organ conserving treatment for cancer , notably and more recently , for carcinoma of the breast , bladder and buccal cavity , in addition to its traditional applications in gynecological and cutaneous cancers .
	manualset3
226240	11	421111	7	NULL	NULL	0	NULL	bladder	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether used alone or in conjunction with surgery and ( or ) external irradiation , brachytherapy has contributed to the development of organ conserving treatment for cancer , notably and more recently , for carcinoma of the breast , bladder and buccal cavity , in addition to its traditional applications in gynecological and cutaneous cancers .
	manualset3
226241	12	421111	7	NULL	NULL	0	NULL	buccal cavity	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether used alone or in conjunction with surgery and ( or ) external irradiation , brachytherapy has contributed to the development of organ conserving treatment for cancer , notably and more recently , for carcinoma of the breast , bladder and buccal cavity , in addition to its traditional applications in gynecological and cutaneous cancers .
	manualset3
226242	13	421111	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether used alone or in conjunction with surgery and ( or ) external irradiation , brachytherapy has contributed to the development of organ conserving treatment for cancer , notably and more recently , for carcinoma of the breast , bladder and buccal cavity , in addition to its traditional applications in gynecological and cutaneous cancers .
	manualset3
226243	14	421111	7	NULL	NULL	0	NULL	traditional applications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether used alone or in conjunction with surgery and ( or ) external irradiation , brachytherapy has contributed to the development of organ conserving treatment for cancer , notably and more recently , for carcinoma of the breast , bladder and buccal cavity , in addition to its traditional applications in gynecological and cutaneous cancers .
	manualset3
226244	15	421111	7	NULL	NULL	0	NULL	 gynecological cancers	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether used alone or in conjunction with surgery and ( or ) external irradiation , brachytherapy has contributed to the development of organ conserving treatment for cancer , notably and more recently , for carcinoma of the breast , bladder and buccal cavity , in addition to its traditional applications in gynecological and cutaneous cancers .
	manualset3
226245	16	421111	7	NULL	NULL	0	NULL	cutaneous cancers 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Whether used alone or in conjunction with surgery and ( or ) external irradiation , brachytherapy has contributed to the development of organ conserving treatment for cancer , notably and more recently , for carcinoma of the breast , bladder and buccal cavity , in addition to its traditional applications in gynecological and cutaneous cancers .
	manualset3
226246	1	421112	7	NULL	NULL	0	NULL	herbicide treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Besides , when the herbicide treatment ( 100 mg 2 , 4-D / kg ) was withdrawn from the dams , 2 , 4-D residues remained in the stomach content of neonates for at least one week .
	manualset3
226247	2	421112	7	NULL	NULL	NULL	NULL	100 mg 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides , when the herbicide treatment ( 100 mg 2 , 4-D / kg ) was withdrawn from the dams , 2 , 4-D residues remained in the stomach content of neonates for at least one week .
	manualset3
226248	3	421112	7	NULL	NULL	0	NULL	2 , 4-D / kg	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Besides , when the herbicide treatment ( 100 mg 2 , 4-D / kg ) was withdrawn from the dams , 2 , 4-D residues remained in the stomach content of neonates for at least one week .
	manualset3
226249	4	421112	7	NULL	NULL	0	NULL	 dams	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Besides , when the herbicide treatment ( 100 mg 2 , 4-D / kg ) was withdrawn from the dams , 2 , 4-D residues remained in the stomach content of neonates for at least one week .
	manualset3
226250	5	421112	7	NULL	NULL	0	NULL	 2 , 4-D residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Besides , when the herbicide treatment ( 100 mg 2 , 4-D / kg ) was withdrawn from the dams , 2 , 4-D residues remained in the stomach content of neonates for at least one week .
	manualset3
226251	6	421112	7	NULL	NULL	0	NULL	stomach content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Besides , when the herbicide treatment ( 100 mg 2 , 4-D / kg ) was withdrawn from the dams , 2 , 4-D residues remained in the stomach content of neonates for at least one week .
	manualset3
226252	7	421112	7	NULL	NULL	0	NULL	 neonates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Besides , when the herbicide treatment ( 100 mg 2 , 4-D / kg ) was withdrawn from the dams , 2 , 4-D residues remained in the stomach content of neonates for at least one week .
	manualset3
226253	8	421112	7	NULL	NULL	0	NULL	one week 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Besides , when the herbicide treatment ( 100 mg 2 , 4-D / kg ) was withdrawn from the dams , 2 , 4-D residues remained in the stomach content of neonates for at least one week .
	manualset3
226254	1	421113	7	NULL	NULL	0	NULL	modified lysines	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these modified lysines , those located in the sequence comprising residues 318-336 ( in the largest human tau isoform ) were found to be glycated , as determined by the reaction with an antibody that recognizes a glycated peptide containing this sequence .
	manualset3
226255	2	421113	7	NULL	NULL	0	NULL	sequence	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these modified lysines , those located in the sequence comprising residues 318-336 ( in the largest human tau isoform ) were found to be glycated , as determined by the reaction with an antibody that recognizes a glycated peptide containing this sequence .
	manualset3
226256	3	421113	7	NULL	NULL	0	NULL	 residues 318-336 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these modified lysines , those located in the sequence comprising residues 318-336 ( in the largest human tau isoform ) were found to be glycated , as determined by the reaction with an antibody that recognizes a glycated peptide containing this sequence .
	manualset3
226257	4	421113	7	NULL	NULL	0	NULL	largest human tau isoform	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these modified lysines , those located in the sequence comprising residues 318-336 ( in the largest human tau isoform ) were found to be glycated , as determined by the reaction with an antibody that recognizes a glycated peptide containing this sequence .
	manualset3
226258	5	421113	7	NULL	NULL	0	NULL	 reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these modified lysines , those located in the sequence comprising residues 318-336 ( in the largest human tau isoform ) were found to be glycated , as determined by the reaction with an antibody that recognizes a glycated peptide containing this sequence .
	manualset3
226259	6	421113	7	NULL	NULL	0	NULL	antibody	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these modified lysines , those located in the sequence comprising residues 318-336 ( in the largest human tau isoform ) were found to be glycated , as determined by the reaction with an antibody that recognizes a glycated peptide containing this sequence .
	manualset3
226260	7	421113	7	NULL	NULL	0	NULL	glycated peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these modified lysines , those located in the sequence comprising residues 318-336 ( in the largest human tau isoform ) were found to be glycated , as determined by the reaction with an antibody that recognizes a glycated peptide containing this sequence .
	manualset3
226261	8	421113	7	NULL	NULL	0	NULL	sequence	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these modified lysines , those located in the sequence comprising residues 318-336 ( in the largest human tau isoform ) were found to be glycated , as determined by the reaction with an antibody that recognizes a glycated peptide containing this sequence .
	manualset3
226262	1	421114	7	NULL	NULL	0	NULL	strain-related responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the strain-related responses they show , is a reduced rate of apoptosis .
	manualset3
226263	2	421114	7	NULL	NULL	0	NULL	reduced rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the strain-related responses they show , is a reduced rate of apoptosis .
	manualset3
226264	3	421114	7	NULL	NULL	0	NULL	 apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the strain-related responses they show , is a reduced rate of apoptosis .
	manualset3
226265	1	421115	7	NULL	NULL	0	NULL	Colourless crystals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Colourless crystals of the title mixed ligand complex , ( Ag ( C ( 5 ) H ( 7 ) N ( 3 ) ) ( C ( 6 ) H ( 9 ) N ( 3 ) ) ) ClO ( 4 ) , were obtained from a solution of 2-amino-4-methyl-pyrimidine , 2-amino-4 , 6 - dimethyl-pyrim-idine and silver perchlorate in water and methanol .
	manualset3
226266	2	421115	7	NULL	NULL	0	NULL	title mixed ligand complex 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Colourless crystals of the title mixed ligand complex , ( Ag ( C ( 5 ) H ( 7 ) N ( 3 ) ) ( C ( 6 ) H ( 9 ) N ( 3 ) ) ) ClO ( 4 ) , were obtained from a solution of 2-amino-4-methyl-pyrimidine , 2-amino-4 , 6 - dimethyl-pyrim-idine and silver perchlorate in water and methanol .
	manualset3
226267	3	421115	7	NULL	NULL	0	NULL	 ( Ag ( C ( 5 ) H ( 7 ) N ( 3 ) ) ( C ( 6 ) H ( 9 ) N ( 3 ) ) ) ClO ( 4 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Colourless crystals of the title mixed ligand complex , ( Ag ( C ( 5 ) H ( 7 ) N ( 3 ) ) ( C ( 6 ) H ( 9 ) N ( 3 ) ) ) ClO ( 4 ) , were obtained from a solution of 2-amino-4-methyl-pyrimidine , 2-amino-4 , 6 - dimethyl-pyrim-idine and silver perchlorate in water and methanol .
	manualset3
226268	4	421115	7	NULL	NULL	0	NULL	solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Colourless crystals of the title mixed ligand complex , ( Ag ( C ( 5 ) H ( 7 ) N ( 3 ) ) ( C ( 6 ) H ( 9 ) N ( 3 ) ) ) ClO ( 4 ) , were obtained from a solution of 2-amino-4-methyl-pyrimidine , 2-amino-4 , 6 - dimethyl-pyrim-idine and silver perchlorate in water and methanol .
	manualset3
226269	5	421115	7	NULL	NULL	0	NULL	2-amino-4-methyl-pyrimidine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Colourless crystals of the title mixed ligand complex , ( Ag ( C ( 5 ) H ( 7 ) N ( 3 ) ) ( C ( 6 ) H ( 9 ) N ( 3 ) ) ) ClO ( 4 ) , were obtained from a solution of 2-amino-4-methyl-pyrimidine , 2-amino-4 , 6 - dimethyl-pyrim-idine and silver perchlorate in water and methanol .
	manualset3
226270	6	421115	7	NULL	NULL	0	NULL	2-amino-4 , 6 - dimethyl-pyrim-idine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Colourless crystals of the title mixed ligand complex , ( Ag ( C ( 5 ) H ( 7 ) N ( 3 ) ) ( C ( 6 ) H ( 9 ) N ( 3 ) ) ) ClO ( 4 ) , were obtained from a solution of 2-amino-4-methyl-pyrimidine , 2-amino-4 , 6 - dimethyl-pyrim-idine and silver perchlorate in water and methanol .
	manualset3
226271	7	421115	7	NULL	NULL	0	NULL	silver perchlorate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Colourless crystals of the title mixed ligand complex , ( Ag ( C ( 5 ) H ( 7 ) N ( 3 ) ) ( C ( 6 ) H ( 9 ) N ( 3 ) ) ) ClO ( 4 ) , were obtained from a solution of 2-amino-4-methyl-pyrimidine , 2-amino-4 , 6 - dimethyl-pyrim-idine and silver perchlorate in water and methanol .
	manualset3
226272	8	421115	7	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Colourless crystals of the title mixed ligand complex , ( Ag ( C ( 5 ) H ( 7 ) N ( 3 ) ) ( C ( 6 ) H ( 9 ) N ( 3 ) ) ) ClO ( 4 ) , were obtained from a solution of 2-amino-4-methyl-pyrimidine , 2-amino-4 , 6 - dimethyl-pyrim-idine and silver perchlorate in water and methanol .
	manualset3
226273	9	421115	7	NULL	NULL	0	NULL	methanol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Colourless crystals of the title mixed ligand complex , ( Ag ( C ( 5 ) H ( 7 ) N ( 3 ) ) ( C ( 6 ) H ( 9 ) N ( 3 ) ) ) ClO ( 4 ) , were obtained from a solution of 2-amino-4-methyl-pyrimidine , 2-amino-4 , 6 - dimethyl-pyrim-idine and silver perchlorate in water and methanol .
	manualset3
226274	1	421116	7	NULL	NULL	0	NULL	Akt3 ( Nmf350 ) mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Akt3 ( Nmf350 ) mice provide a new tool for studying physiological roles of AKT signaling in the brain , and potentially novel mechanisms for epilepsy .
	manualset3
226275	2	421116	7	NULL	NULL	NULL	NULL	new tool	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Akt3 ( Nmf350 ) mice provide a new tool for studying physiological roles of AKT signaling in the brain , and potentially novel mechanisms for epilepsy .
	manualset3
226276	3	421116	7	NULL	NULL	0	NULL	physiological roles 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Akt3 ( Nmf350 ) mice provide a new tool for studying physiological roles of AKT signaling in the brain , and potentially novel mechanisms for epilepsy .
	manualset3
226277	4	421116	7	NULL	NULL	0	NULL	AKT signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Akt3 ( Nmf350 ) mice provide a new tool for studying physiological roles of AKT signaling in the brain , and potentially novel mechanisms for epilepsy .
	manualset3
226278	5	421116	7	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Akt3 ( Nmf350 ) mice provide a new tool for studying physiological roles of AKT signaling in the brain , and potentially novel mechanisms for epilepsy .
	manualset3
226279	6	421116	7	NULL	NULL	0	NULL	novel mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Akt3 ( Nmf350 ) mice provide a new tool for studying physiological roles of AKT signaling in the brain , and potentially novel mechanisms for epilepsy .
	manualset3
226280	7	421116	7	NULL	NULL	0	NULL	epilepsy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Akt3 ( Nmf350 ) mice provide a new tool for studying physiological roles of AKT signaling in the brain , and potentially novel mechanisms for epilepsy .
	manualset3
226281	1	421117	7	NULL	NULL	0	NULL	method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Our method of injury involved a surgical model with identical partial lacerations in the midsubstance of the MCL and ACL .
	manualset3
226282	2	421117	7	NULL	NULL	0	NULL	injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our method of injury involved a surgical model with identical partial lacerations in the midsubstance of the MCL and ACL .
	manualset3
226283	3	421117	7	NULL	NULL	0	NULL	surgical model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Our method of injury involved a surgical model with identical partial lacerations in the midsubstance of the MCL and ACL .
	manualset3
226284	4	421117	7	NULL	NULL	0	NULL	 identical partial lacerations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our method of injury involved a surgical model with identical partial lacerations in the midsubstance of the MCL and ACL .
	manualset3
226285	5	421117	7	NULL	NULL	0	NULL	midsubstance	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our method of injury involved a surgical model with identical partial lacerations in the midsubstance of the MCL and ACL .
	manualset3
226286	6	421117	7	NULL	NULL	0	NULL	 MCL	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our method of injury involved a surgical model with identical partial lacerations in the midsubstance of the MCL and ACL .
	manualset3
226287	7	421117	7	NULL	NULL	0	NULL	ACL	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Our method of injury involved a surgical model with identical partial lacerations in the midsubstance of the MCL and ACL .
	manualset3
226288	1	421118	7	NULL	NULL	0	NULL	Identification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of PA-derived telomere-related restriction fragments will enable further genetic analysis of this region of the mouse genome .
	manualset3
226289	2	421118	7	NULL	NULL	0	NULL	PA-derived telomere-related restriction fragments	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of PA-derived telomere-related restriction fragments will enable further genetic analysis of this region of the mouse genome .
	manualset3
226290	3	421118	7	NULL	NULL	0	NULL	genetic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of PA-derived telomere-related restriction fragments will enable further genetic analysis of this region of the mouse genome .
	manualset3
226291	4	421118	7	NULL	NULL	0	NULL	 region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of PA-derived telomere-related restriction fragments will enable further genetic analysis of this region of the mouse genome .
	manualset3
226292	5	421118	7	NULL	NULL	0	NULL	mouse genome	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Identification of PA-derived telomere-related restriction fragments will enable further genetic analysis of this region of the mouse genome .
	manualset3
226293	1	421119	7	NULL	NULL	NULL	NULL	center crystal	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The center crystal , placed at the perfusion boundary ( PB ) between left anterior descending and circumflex arteries , radiated ultrasound to receiver crystals 7-17 mm to either side of the PB .
	manualset3
226294	2	421119	7	NULL	NULL	0	NULL	perfusion boundary ( PB )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The center crystal , placed at the perfusion boundary ( PB ) between left anterior descending and circumflex arteries , radiated ultrasound to receiver crystals 7-17 mm to either side of the PB .
	manualset3
226295	3	421119	7	NULL	NULL	0	NULL	left anterior descending arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The center crystal , placed at the perfusion boundary ( PB ) between left anterior descending and circumflex arteries , radiated ultrasound to receiver crystals 7-17 mm to either side of the PB .
	manualset3
226296	4	421119	7	NULL	NULL	0	NULL	circumflex arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The center crystal , placed at the perfusion boundary ( PB ) between left anterior descending and circumflex arteries , radiated ultrasound to receiver crystals 7-17 mm to either side of the PB .
	manualset3
226297	5	421119	7	NULL	NULL	0	NULL	ultrasound 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The center crystal , placed at the perfusion boundary ( PB ) between left anterior descending and circumflex arteries , radiated ultrasound to receiver crystals 7-17 mm to either side of the PB .
	manualset3
226298	6	421119	7	NULL	NULL	0	NULL	crystals 7-17 mm	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The center crystal , placed at the perfusion boundary ( PB ) between left anterior descending and circumflex arteries , radiated ultrasound to receiver crystals 7-17 mm to either side of the PB .
	manualset3
226299	7	421119	7	NULL	NULL	0	NULL	side of the PB 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The center crystal , placed at the perfusion boundary ( PB ) between left anterior descending and circumflex arteries , radiated ultrasound to receiver crystals 7-17 mm to either side of the PB .
	manualset3
226300	1	421120	7	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of PDBu , adenosine ( 10-5 M ) still hyperpolarized membrane voltage of mesangial cells .6 .
	manualset3
226301	2	421120	7	NULL	NULL	0	NULL	PDBu	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of PDBu , adenosine ( 10-5 M ) still hyperpolarized membrane voltage of mesangial cells .6 .
	manualset3
226302	3	421120	7	NULL	NULL	0	NULL	adenosine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of PDBu , adenosine ( 10-5 M ) still hyperpolarized membrane voltage of mesangial cells .6 .
	manualset3
226303	4	421120	7	NULL	NULL	0	NULL	10-5 M 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of PDBu , adenosine ( 10-5 M ) still hyperpolarized membrane voltage of mesangial cells .6 .
	manualset3
226304	5	421120	7	NULL	NULL	0	NULL	membrane voltage 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of PDBu , adenosine ( 10-5 M ) still hyperpolarized membrane voltage of mesangial cells .6 .
	manualset3
226305	6	421120	7	NULL	NULL	0	NULL	mesangial cells .6 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of PDBu , adenosine ( 10-5 M ) still hyperpolarized membrane voltage of mesangial cells .6 .
	manualset3
226531	1	421121	7	NULL	NULL	0	NULL	Dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dysfunction of fistulae is the most common reason for a second intervention and recurrent hospitalization .
	manualset3
226612	2	421121	7	NULL	NULL	0	NULL	fistulae 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Dysfunction of fistulae is the most common reason for a second intervention and recurrent hospitalization .
	manualset3
226613	3	421121	7	NULL	NULL	0	NULL	reason	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dysfunction of fistulae is the most common reason for a second intervention and recurrent hospitalization .
	manualset3
226614	4	421121	7	NULL	NULL	0	NULL	second intervention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Dysfunction of fistulae is the most common reason for a second intervention and recurrent hospitalization .
	manualset3
226615	5	421121	7	NULL	NULL	0	NULL	 recurrent hospitalization .	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Dysfunction of fistulae is the most common reason for a second intervention and recurrent hospitalization .
	manualset3
226616	1	421122	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we will describe these issues , including induced dependent censoring and limited identifiability with the cost distribution , and review recent statistical developments .
	manualset3
226617	2	421122	7	NULL	NULL	0	NULL	issues	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we will describe these issues , including induced dependent censoring and limited identifiability with the cost distribution , and review recent statistical developments .
	manualset3
226618	3	421122	7	NULL	NULL	0	NULL	induced dependent censoring	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we will describe these issues , including induced dependent censoring and limited identifiability with the cost distribution , and review recent statistical developments .
	manualset3
226619	4	421122	7	NULL	NULL	0	NULL	limited identifiability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we will describe these issues , including induced dependent censoring and limited identifiability with the cost distribution , and review recent statistical developments .
	manualset3
226620	5	421122	7	NULL	NULL	0	NULL	cost distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we will describe these issues , including induced dependent censoring and limited identifiability with the cost distribution , and review recent statistical developments .
	manualset3
226621	6	421122	7	NULL	NULL	0	NULL	statistical developments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this article , we will describe these issues , including induced dependent censoring and limited identifiability with the cost distribution , and review recent statistical developments .
	manualset3
226622	1	421123	7	NULL	NULL	0	NULL	Cytomegalovirus Retinitis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The Cytomegalovirus Retinitis and Viral Resistance Study Group .
	manualset3
226623	2	421123	7	NULL	NULL	0	NULL	Viral Resistance Study Group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The Cytomegalovirus Retinitis and Viral Resistance Study Group .
	manualset3
226624	1	421124	7	NULL	NULL	0	NULL	No renal injury 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No renal injury was detected in the 88 infants and children with lower symptomatic urinary tract infection or asymptomatic bacteriuria .
	manualset3
226625	2	421124	7	NULL	NULL	0	NULL	88 infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No renal injury was detected in the 88 infants and children with lower symptomatic urinary tract infection or asymptomatic bacteriuria .
	manualset3
226626	3	421124	7	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	No renal injury was detected in the 88 infants and children with lower symptomatic urinary tract infection or asymptomatic bacteriuria .
	manualset3
226627	4	421124	7	NULL	NULL	0	NULL	 lower symptomatic urinary tract infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No renal injury was detected in the 88 infants and children with lower symptomatic urinary tract infection or asymptomatic bacteriuria .
	manualset3
226628	5	421124	7	NULL	NULL	0	NULL	asymptomatic bacteriuria 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No renal injury was detected in the 88 infants and children with lower symptomatic urinary tract infection or asymptomatic bacteriuria .
	manualset3
226629	1	421125	7	NULL	NULL	0	NULL	 alpha-adrenergic blocking agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using alpha-adrenergic blocking agents , the smooth muscle contribution to the maximum urethral pressure was ascertained in each group and differences in both the configuration of the profile , and the smooth muscle component , were found .
	manualset3
226630	2	421125	7	NULL	NULL	NULL	NULL	smooth muscle contribution	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Using alpha-adrenergic blocking agents , the smooth muscle contribution to the maximum urethral pressure was ascertained in each group and differences in both the configuration of the profile , and the smooth muscle component , were found .
	manualset3
226631	3	421125	7	NULL	NULL	0	NULL	maximum urethral pressure 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using alpha-adrenergic blocking agents , the smooth muscle contribution to the maximum urethral pressure was ascertained in each group and differences in both the configuration of the profile , and the smooth muscle component , were found .
	manualset3
226632	4	421125	7	NULL	NULL	0	NULL	each group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using alpha-adrenergic blocking agents , the smooth muscle contribution to the maximum urethral pressure was ascertained in each group and differences in both the configuration of the profile , and the smooth muscle component , were found .
	manualset3
226633	5	421125	7	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Using alpha-adrenergic blocking agents , the smooth muscle contribution to the maximum urethral pressure was ascertained in each group and differences in both the configuration of the profile , and the smooth muscle component , were found .
	manualset3
226634	6	421125	7	NULL	NULL	0	NULL	configuration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using alpha-adrenergic blocking agents , the smooth muscle contribution to the maximum urethral pressure was ascertained in each group and differences in both the configuration of the profile , and the smooth muscle component , were found .
	manualset3
226635	7	421125	7	NULL	NULL	0	NULL	profile	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using alpha-adrenergic blocking agents , the smooth muscle contribution to the maximum urethral pressure was ascertained in each group and differences in both the configuration of the profile , and the smooth muscle component , were found .
	manualset3
226636	8	421125	7	NULL	NULL	0	NULL	smooth muscle component	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Using alpha-adrenergic blocking agents , the smooth muscle contribution to the maximum urethral pressure was ascertained in each group and differences in both the configuration of the profile , and the smooth muscle component , were found .
	manualset3
226637	1	421126	7	NULL	NULL	NULL	NULL	state 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Intriguingly , such a state was not found in a cavity-filling mutant of WT ( S ) , C130I/V103L , suggesting that this state is mediated by cavity hydration .
	manualset3
226638	2	421126	7	NULL	NULL	0	NULL	cavity-filling mutant	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Intriguingly , such a state was not found in a cavity-filling mutant of WT ( S ) , C130I/V103L , suggesting that this state is mediated by cavity hydration .
	manualset3
226639	3	421126	7	NULL	NULL	0	NULL	WT ( S )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Intriguingly , such a state was not found in a cavity-filling mutant of WT ( S ) , C130I/V103L , suggesting that this state is mediated by cavity hydration .
	manualset3
226640	4	421126	7	NULL	NULL	0	NULL	C130I/V103L	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Intriguingly , such a state was not found in a cavity-filling mutant of WT ( S ) , C130I/V103L , suggesting that this state is mediated by cavity hydration .
	manualset3
226641	5	421126	7	NULL	NULL	0	NULL	state	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Intriguingly , such a state was not found in a cavity-filling mutant of WT ( S ) , C130I/V103L , suggesting that this state is mediated by cavity hydration .
	manualset3
226642	6	421126	7	NULL	NULL	0	NULL	cavity hydration	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intriguingly , such a state was not found in a cavity-filling mutant of WT ( S ) , C130I/V103L , suggesting that this state is mediated by cavity hydration .
	manualset3
226643	1	421127	7	NULL	NULL	0	NULL	Determination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of chloramphenicol cinnamate by rapid polarography in a syrup with a complex formulation and in the presence of reductants ) .
	manualset3
226644	2	421127	7	NULL	NULL	0	NULL	chloramphenicol cinnamate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of chloramphenicol cinnamate by rapid polarography in a syrup with a complex formulation and in the presence of reductants ) .
	manualset3
226645	3	421127	7	NULL	NULL	0	NULL	 rapid polarography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of chloramphenicol cinnamate by rapid polarography in a syrup with a complex formulation and in the presence of reductants ) .
	manualset3
226646	4	421127	7	NULL	NULL	0	NULL	syrup	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of chloramphenicol cinnamate by rapid polarography in a syrup with a complex formulation and in the presence of reductants ) .
	manualset3
226647	5	421127	7	NULL	NULL	0	NULL	complex formulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of chloramphenicol cinnamate by rapid polarography in a syrup with a complex formulation and in the presence of reductants ) .
	manualset3
226648	6	421127	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of chloramphenicol cinnamate by rapid polarography in a syrup with a complex formulation and in the presence of reductants ) .
	manualset3
226649	7	421127	7	NULL	NULL	0	NULL	 reductants	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of chloramphenicol cinnamate by rapid polarography in a syrup with a complex formulation and in the presence of reductants ) .
	manualset3
226650	1	421128	7	NULL	NULL	0	NULL	areas	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	All other areas differed between milk in both VE and total dust endotoxin burdens .
	manualset3
226651	2	421128	7	NULL	NULL	0	NULL	milk	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All other areas differed between milk in both VE and total dust endotoxin burdens .
	manualset3
226652	3	421128	7	NULL	NULL	0	NULL	VE	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	All other areas differed between milk in both VE and total dust endotoxin burdens .
	manualset3
226653	4	421128	7	NULL	NULL	0	NULL	total dust endotoxin burdens	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All other areas differed between milk in both VE and total dust endotoxin burdens .
	manualset3
226654	1	421129	7	NULL	NULL	NULL	NULL	malignant tumor	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A malignant tumor may require withdrawal of immunosuppressive therapy and removal of the transplanted organ , whereas a benign cyst would require no therapy unless it becomes infected or produces obstruction .
	manualset3
226655	2	421129	7	NULL	NULL	0	NULL	 withdrawal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A malignant tumor may require withdrawal of immunosuppressive therapy and removal of the transplanted organ , whereas a benign cyst would require no therapy unless it becomes infected or produces obstruction .
	manualset3
226656	3	421129	7	NULL	NULL	0	NULL	 immunosuppressive therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A malignant tumor may require withdrawal of immunosuppressive therapy and removal of the transplanted organ , whereas a benign cyst would require no therapy unless it becomes infected or produces obstruction .
	manualset3
226657	4	421129	7	NULL	NULL	0	NULL	 removal	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A malignant tumor may require withdrawal of immunosuppressive therapy and removal of the transplanted organ , whereas a benign cyst would require no therapy unless it becomes infected or produces obstruction .
	manualset3
226658	5	421129	7	NULL	NULL	0	NULL	transplanted organ	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A malignant tumor may require withdrawal of immunosuppressive therapy and removal of the transplanted organ , whereas a benign cyst would require no therapy unless it becomes infected or produces obstruction .
	manualset3
226659	6	421129	7	NULL	NULL	NULL	NULL	benign cyst 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A malignant tumor may require withdrawal of immunosuppressive therapy and removal of the transplanted organ , whereas a benign cyst would require no therapy unless it becomes infected or produces obstruction .
	manualset3
226660	7	421129	7	NULL	NULL	0	NULL	no therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A malignant tumor may require withdrawal of immunosuppressive therapy and removal of the transplanted organ , whereas a benign cyst would require no therapy unless it becomes infected or produces obstruction .
	manualset3
226661	8	421129	7	NULL	NULL	NULL	NULL	obstruction	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A malignant tumor may require withdrawal of immunosuppressive therapy and removal of the transplanted organ , whereas a benign cyst would require no therapy unless it becomes infected or produces obstruction .
	manualset3
226662	1	421130	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of SF I , V of the DNA-polymerizing reaction was increased and Km values for the substrates of this reaction were not changed .
	manualset3
226663	2	421130	7	NULL	NULL	0	NULL	SF I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of SF I , V of the DNA-polymerizing reaction was increased and Km values for the substrates of this reaction were not changed .
	manualset3
226664	3	421130	7	NULL	NULL	0	NULL	V 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of SF I , V of the DNA-polymerizing reaction was increased and Km values for the substrates of this reaction were not changed .
	manualset3
226665	4	421130	7	NULL	NULL	0	NULL	DNA-polymerizing reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of SF I , V of the DNA-polymerizing reaction was increased and Km values for the substrates of this reaction were not changed .
	manualset3
226666	5	421130	7	NULL	NULL	0	NULL	Km values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of SF I , V of the DNA-polymerizing reaction was increased and Km values for the substrates of this reaction were not changed .
	manualset3
226667	6	421130	7	NULL	NULL	0	NULL	 substrates	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of SF I , V of the DNA-polymerizing reaction was increased and Km values for the substrates of this reaction were not changed .
	manualset3
226668	7	421130	7	NULL	NULL	0	NULL	 reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the presence of SF I , V of the DNA-polymerizing reaction was increased and Km values for the substrates of this reaction were not changed .
	manualset3
226669	1	421131	7	NULL	NULL	0	NULL	Hepatocellular damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Hepatocellular damage during pneumonia ) .
	manualset3
226670	2	421131	7	NULL	NULL	0	NULL	pneumonia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Hepatocellular damage during pneumonia ) .
	manualset3
226746	1	421132	7	NULL	NULL	0	NULL	 period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , increasing the period of hypovolemia produced further decreases in pancreatic flow and bicarbonate secretion only .
	manualset3
226747	2	421132	7	NULL	NULL	0	NULL	hypovolemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , increasing the period of hypovolemia produced further decreases in pancreatic flow and bicarbonate secretion only .
	manualset3
226748	3	421132	7	NULL	NULL	0	NULL	pancreatic flow	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , increasing the period of hypovolemia produced further decreases in pancreatic flow and bicarbonate secretion only .
	manualset3
226749	4	421132	7	NULL	NULL	0	NULL	 bicarbonate secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , increasing the period of hypovolemia produced further decreases in pancreatic flow and bicarbonate secretion only .
	manualset3
226750	1	421133	7	NULL	NULL	0	NULL	first group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The first group consisted of 242 non-goitrous subjects , and the second , contained 603 subjects with different grades of goiter .
	manualset3
226751	2	421133	7	NULL	NULL	0	NULL	242 non-goitrous subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The first group consisted of 242 non-goitrous subjects , and the second , contained 603 subjects with different grades of goiter .
	manualset3
226752	3	421133	7	NULL	NULL	0	NULL	 second group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The first group consisted of 242 non-goitrous subjects , and the second , contained 603 subjects with different grades of goiter .
	manualset3
226753	4	421133	7	NULL	NULL	0	NULL	603 subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The first group consisted of 242 non-goitrous subjects , and the second , contained 603 subjects with different grades of goiter .
	manualset3
226754	5	421133	7	NULL	NULL	0	NULL	different grades	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The first group consisted of 242 non-goitrous subjects , and the second , contained 603 subjects with different grades of goiter .
	manualset3
226755	6	421133	7	NULL	NULL	0	NULL	goiter	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The first group consisted of 242 non-goitrous subjects , and the second , contained 603 subjects with different grades of goiter .
	manualset3
226756	1	421134	7	NULL	NULL	0	NULL	All trans retinoic acid ( ATRA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All trans retinoic acid ( ATRA ) in the treatment of acute promyelocytic leukemia is the first model of differentiation therapy in malignancies , and represents the first strict correlation between a genetic defect and a specific treatment .
	manualset3
226757	2	421134	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All trans retinoic acid ( ATRA ) in the treatment of acute promyelocytic leukemia is the first model of differentiation therapy in malignancies , and represents the first strict correlation between a genetic defect and a specific treatment .
	manualset3
226758	3	421134	7	NULL	NULL	0	NULL	acute promyelocytic leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	All trans retinoic acid ( ATRA ) in the treatment of acute promyelocytic leukemia is the first model of differentiation therapy in malignancies , and represents the first strict correlation between a genetic defect and a specific treatment .
	manualset3
226759	4	421134	7	NULL	NULL	0	NULL	first model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	All trans retinoic acid ( ATRA ) in the treatment of acute promyelocytic leukemia is the first model of differentiation therapy in malignancies , and represents the first strict correlation between a genetic defect and a specific treatment .
	manualset3
226760	5	421134	7	NULL	NULL	0	NULL	differentiation therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All trans retinoic acid ( ATRA ) in the treatment of acute promyelocytic leukemia is the first model of differentiation therapy in malignancies , and represents the first strict correlation between a genetic defect and a specific treatment .
	manualset3
226761	6	421134	7	NULL	NULL	0	NULL	first strict correlation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	All trans retinoic acid ( ATRA ) in the treatment of acute promyelocytic leukemia is the first model of differentiation therapy in malignancies , and represents the first strict correlation between a genetic defect and a specific treatment .
	manualset3
226762	7	421134	7	NULL	NULL	0	NULL	genetic defect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All trans retinoic acid ( ATRA ) in the treatment of acute promyelocytic leukemia is the first model of differentiation therapy in malignancies , and represents the first strict correlation between a genetic defect and a specific treatment .
	manualset3
226763	8	421134	7	NULL	NULL	0	NULL	specific treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All trans retinoic acid ( ATRA ) in the treatment of acute promyelocytic leukemia is the first model of differentiation therapy in malignancies , and represents the first strict correlation between a genetic defect and a specific treatment .
	manualset3
228649	9	421134	7	NULL	NULL	0	NULL	malignancies	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	All trans retinoic acid ( ATRA ) in the treatment of acute promyelocytic leukemia is the first model of differentiation therapy in malignancies , and represents the first strict correlation between a genetic defect and a specific treatment .
	manualset3
226764	1	421135	7	NULL	NULL	0	NULL	 case 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The case is presented to sensitize the physicians to keep malaria as a differential in cases of fever with purpura fulminans .
	manualset3
226765	2	421135	7	NULL	NULL	0	NULL	 physicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The case is presented to sensitize the physicians to keep malaria as a differential in cases of fever with purpura fulminans .
	manualset3
226766	3	421135	7	NULL	NULL	0	NULL	malaria	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The case is presented to sensitize the physicians to keep malaria as a differential in cases of fever with purpura fulminans .
	manualset3
226767	4	421135	7	NULL	NULL	0	NULL	cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The case is presented to sensitize the physicians to keep malaria as a differential in cases of fever with purpura fulminans .
	manualset3
226768	5	421135	7	NULL	NULL	0	NULL	 fever	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The case is presented to sensitize the physicians to keep malaria as a differential in cases of fever with purpura fulminans .
	manualset3
226769	6	421135	7	NULL	NULL	0	NULL	purpura fulminans	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The case is presented to sensitize the physicians to keep malaria as a differential in cases of fever with purpura fulminans .
	manualset3
226770	1	421136	7	NULL	NULL	0	NULL	STAT1	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	This suggests that STAT1 regulates expression of gene ( s ) involved in cell surface trafficking of Fas in response to CPT-11 or tomudex .
	manualset3
226771	2	421136	7	NULL	NULL	0	NULL	 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This suggests that STAT1 regulates expression of gene ( s ) involved in cell surface trafficking of Fas in response to CPT-11 or tomudex .
	manualset3
226772	3	421136	7	NULL	NULL	0	NULL	gene ( s )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This suggests that STAT1 regulates expression of gene ( s ) involved in cell surface trafficking of Fas in response to CPT-11 or tomudex .
	manualset3
226773	4	421136	7	NULL	NULL	0	NULL	cell surface trafficking 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This suggests that STAT1 regulates expression of gene ( s ) involved in cell surface trafficking of Fas in response to CPT-11 or tomudex .
	manualset3
226774	5	421136	7	NULL	NULL	0	NULL	Fas 	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	This suggests that STAT1 regulates expression of gene ( s ) involved in cell surface trafficking of Fas in response to CPT-11 or tomudex .
	manualset3
226775	6	421136	7	NULL	NULL	0	NULL	CPT-11 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	This suggests that STAT1 regulates expression of gene ( s ) involved in cell surface trafficking of Fas in response to CPT-11 or tomudex .
	manualset3
226776	7	421136	7	NULL	NULL	0	NULL	tomudex	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	This suggests that STAT1 regulates expression of gene ( s ) involved in cell surface trafficking of Fas in response to CPT-11 or tomudex .
	manualset3
226777	1	421137	7	NULL	NULL	0	NULL	Radiofrequency ablation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiofrequency ablation in the treatment of hepatocellular carcinoma : the need for centralization .
	manualset3
226778	2	421137	7	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiofrequency ablation in the treatment of hepatocellular carcinoma : the need for centralization .
	manualset3
226779	3	421137	7	NULL	NULL	0	NULL	hepatocellular carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiofrequency ablation in the treatment of hepatocellular carcinoma : the need for centralization .
	manualset3
226780	4	421137	7	NULL	NULL	0	NULL	need	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiofrequency ablation in the treatment of hepatocellular carcinoma : the need for centralization .
	manualset3
226781	5	421137	7	NULL	NULL	0	NULL	centralization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiofrequency ablation in the treatment of hepatocellular carcinoma : the need for centralization .
	manualset3
226782	1	421138	7	NULL	NULL	0	NULL	 ten phosphorylated proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these ten phosphorylated proteins , we identified a major cytoplasmic polypeptide ( Mr approximately 64 , 000 ) , a cytoskeletal protein ( Mr approximately 56 , 000 ) , a nonmuscle myosin light chain , and two proteins ( Mr approximately 60 , 000 and 64 , 000 ) localized in or around the cell nucleus .
	manualset3
226783	2	421138	7	NULL	NULL	0	NULL	major cytoplasmic polypeptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these ten phosphorylated proteins , we identified a major cytoplasmic polypeptide ( Mr approximately 64 , 000 ) , a cytoskeletal protein ( Mr approximately 56 , 000 ) , a nonmuscle myosin light chain , and two proteins ( Mr approximately 60 , 000 and 64 , 000 ) localized in or around the cell nucleus .
	manualset3
226784	3	421138	7	NULL	NULL	0	NULL	Mr	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these ten phosphorylated proteins , we identified a major cytoplasmic polypeptide ( Mr approximately 64 , 000 ) , a cytoskeletal protein ( Mr approximately 56 , 000 ) , a nonmuscle myosin light chain , and two proteins ( Mr approximately 60 , 000 and 64 , 000 ) localized in or around the cell nucleus .
	manualset3
226785	4	421138	7	NULL	NULL	0	NULL	64 , 000	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these ten phosphorylated proteins , we identified a major cytoplasmic polypeptide ( Mr approximately 64 , 000 ) , a cytoskeletal protein ( Mr approximately 56 , 000 ) , a nonmuscle myosin light chain , and two proteins ( Mr approximately 60 , 000 and 64 , 000 ) localized in or around the cell nucleus .
	manualset3
226786	5	421138	7	NULL	NULL	0	NULL	cytoskeletal protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these ten phosphorylated proteins , we identified a major cytoplasmic polypeptide ( Mr approximately 64 , 000 ) , a cytoskeletal protein ( Mr approximately 56 , 000 ) , a nonmuscle myosin light chain , and two proteins ( Mr approximately 60 , 000 and 64 , 000 ) localized in or around the cell nucleus .
	manualset3
226787	6	421138	7	NULL	NULL	0	NULL	Mr	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these ten phosphorylated proteins , we identified a major cytoplasmic polypeptide ( Mr approximately 64 , 000 ) , a cytoskeletal protein ( Mr approximately 56 , 000 ) , a nonmuscle myosin light chain , and two proteins ( Mr approximately 60 , 000 and 64 , 000 ) localized in or around the cell nucleus .
	manualset3
226788	7	421138	7	NULL	NULL	0	NULL	56 , 000 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these ten phosphorylated proteins , we identified a major cytoplasmic polypeptide ( Mr approximately 64 , 000 ) , a cytoskeletal protein ( Mr approximately 56 , 000 ) , a nonmuscle myosin light chain , and two proteins ( Mr approximately 60 , 000 and 64 , 000 ) localized in or around the cell nucleus .
	manualset3
226789	8	421138	7	NULL	NULL	0	NULL	nonmuscle myosin light chain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these ten phosphorylated proteins , we identified a major cytoplasmic polypeptide ( Mr approximately 64 , 000 ) , a cytoskeletal protein ( Mr approximately 56 , 000 ) , a nonmuscle myosin light chain , and two proteins ( Mr approximately 60 , 000 and 64 , 000 ) localized in or around the cell nucleus .
	manualset3
226790	9	421138	7	NULL	NULL	0	NULL	two proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these ten phosphorylated proteins , we identified a major cytoplasmic polypeptide ( Mr approximately 64 , 000 ) , a cytoskeletal protein ( Mr approximately 56 , 000 ) , a nonmuscle myosin light chain , and two proteins ( Mr approximately 60 , 000 and 64 , 000 ) localized in or around the cell nucleus .
	manualset3
226791	10	421138	7	NULL	NULL	0	NULL	Mr	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these ten phosphorylated proteins , we identified a major cytoplasmic polypeptide ( Mr approximately 64 , 000 ) , a cytoskeletal protein ( Mr approximately 56 , 000 ) , a nonmuscle myosin light chain , and two proteins ( Mr approximately 60 , 000 and 64 , 000 ) localized in or around the cell nucleus .
	manualset3
226792	11	421138	7	NULL	NULL	0	NULL	60 , 000 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these ten phosphorylated proteins , we identified a major cytoplasmic polypeptide ( Mr approximately 64 , 000 ) , a cytoskeletal protein ( Mr approximately 56 , 000 ) , a nonmuscle myosin light chain , and two proteins ( Mr approximately 60 , 000 and 64 , 000 ) localized in or around the cell nucleus .
	manualset3
226793	12	421138	7	NULL	NULL	0	NULL	 64 , 000	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these ten phosphorylated proteins , we identified a major cytoplasmic polypeptide ( Mr approximately 64 , 000 ) , a cytoskeletal protein ( Mr approximately 56 , 000 ) , a nonmuscle myosin light chain , and two proteins ( Mr approximately 60 , 000 and 64 , 000 ) localized in or around the cell nucleus .
	manualset3
226794	13	421138	7	NULL	NULL	0	NULL	cell nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Among these ten phosphorylated proteins , we identified a major cytoplasmic polypeptide ( Mr approximately 64 , 000 ) , a cytoskeletal protein ( Mr approximately 56 , 000 ) , a nonmuscle myosin light chain , and two proteins ( Mr approximately 60 , 000 and 64 , 000 ) localized in or around the cell nucleus .
	manualset3
226795	1	421139	7	NULL	NULL	0	NULL	Monoclonal antibody ( MAb ) 667	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibody ( MAb ) 667 is a neutralizing mouse monoclonal antibody recognizing the envelope glycoprotein ( Env ) of the ecotropic neurotropic murine retrovirus CasBrE but not that of other murine retroviruses .
	manualset3
226796	2	421139	7	NULL	NULL	0	NULL	neutralizing mouse monoclonal antibody	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibody ( MAb ) 667 is a neutralizing mouse monoclonal antibody recognizing the envelope glycoprotein ( Env ) of the ecotropic neurotropic murine retrovirus CasBrE but not that of other murine retroviruses .
	manualset3
226797	3	421139	7	NULL	NULL	0	NULL	envelope glycoprotein ( Env )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibody ( MAb ) 667 is a neutralizing mouse monoclonal antibody recognizing the envelope glycoprotein ( Env ) of the ecotropic neurotropic murine retrovirus CasBrE but not that of other murine retroviruses .
	manualset3
226798	4	421139	7	NULL	NULL	0	NULL	 ecotropic neurotropic murine retrovirus CasBrE	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibody ( MAb ) 667 is a neutralizing mouse monoclonal antibody recognizing the envelope glycoprotein ( Env ) of the ecotropic neurotropic murine retrovirus CasBrE but not that of other murine retroviruses .
	manualset3
226799	5	421139	7	NULL	NULL	0	NULL	murine retroviruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Monoclonal antibody ( MAb ) 667 is a neutralizing mouse monoclonal antibody recognizing the envelope glycoprotein ( Env ) of the ecotropic neurotropic murine retrovirus CasBrE but not that of other murine retroviruses .
	manualset3
226800	1	421140	7	NULL	NULL	0	NULL	echocardiogram 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	His echocardiogram showed a massive pericardial effusion .
	manualset3
226801	2	421140	7	NULL	NULL	0	NULL	massive pericardial effusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	His echocardiogram showed a massive pericardial effusion .
	manualset3
226881	1	421141	7	NULL	NULL	0	NULL	Recent progresses 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent progresses of magnetic resonance imaging provide new tools to examine in vivo rodent central nervous system , and eventually to monitor the progression of lesions .
	manualset3
226882	2	421141	7	NULL	NULL	0	NULL	magnetic resonance imaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent progresses of magnetic resonance imaging provide new tools to examine in vivo rodent central nervous system , and eventually to monitor the progression of lesions .
	manualset3
226883	3	421141	7	NULL	NULL	0	NULL	new tools 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent progresses of magnetic resonance imaging provide new tools to examine in vivo rodent central nervous system , and eventually to monitor the progression of lesions .
	manualset3
226884	4	421141	7	NULL	NULL	0	NULL	 in vivo rodent central nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent progresses of magnetic resonance imaging provide new tools to examine in vivo rodent central nervous system , and eventually to monitor the progression of lesions .
	manualset3
226885	5	421141	7	NULL	NULL	0	NULL	progression 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent progresses of magnetic resonance imaging provide new tools to examine in vivo rodent central nervous system , and eventually to monitor the progression of lesions .
	manualset3
226886	6	421141	7	NULL	NULL	0	NULL	lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent progresses of magnetic resonance imaging provide new tools to examine in vivo rodent central nervous system , and eventually to monitor the progression of lesions .
	manualset3
226887	1	421142	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient had undergone extirpation of rectal cancer four years previously .
	manualset3
226888	2	421142	7	NULL	NULL	0	NULL	extirpation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient had undergone extirpation of rectal cancer four years previously .
	manualset3
226889	3	421142	7	NULL	NULL	0	NULL	rectal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient had undergone extirpation of rectal cancer four years previously .
	manualset3
226890	4	421142	7	NULL	NULL	0	NULL	four years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient had undergone extirpation of rectal cancer four years previously .
	manualset3
226891	1	421143	7	NULL	NULL	0	NULL	Nitrous oxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitrous oxide becomes the vice of dentists .
	manualset3
226892	2	421143	7	NULL	NULL	0	NULL	 vice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitrous oxide becomes the vice of dentists .
	manualset3
226893	3	421143	7	NULL	NULL	0	NULL	dentists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nitrous oxide becomes the vice of dentists .
	manualset3
226894	1	421144	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide evidence that the protein phosphatase LePS2 ; 1 , plays an important role in phosphate starvation induced processes in tomato .
	manualset3
226895	2	421144	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide evidence that the protein phosphatase LePS2 ; 1 , plays an important role in phosphate starvation induced processes in tomato .
	manualset3
226896	3	421144	7	NULL	NULL	0	NULL	protein phosphatase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide evidence that the protein phosphatase LePS2 ; 1 , plays an important role in phosphate starvation induced processes in tomato .
	manualset3
226897	4	421144	7	NULL	NULL	0	NULL	LePS2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide evidence that the protein phosphatase LePS2 ; 1 , plays an important role in phosphate starvation induced processes in tomato .
	manualset3
226898	5	421144	7	NULL	NULL	0	NULL	role 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide evidence that the protein phosphatase LePS2 ; 1 , plays an important role in phosphate starvation induced processes in tomato .
	manualset3
226899	6	421144	7	NULL	NULL	0	NULL	phosphate starvation induced processes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide evidence that the protein phosphatase LePS2 ; 1 , plays an important role in phosphate starvation induced processes in tomato .
	manualset3
226900	7	421144	7	NULL	NULL	0	NULL	tomato	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide evidence that the protein phosphatase LePS2 ; 1 , plays an important role in phosphate starvation induced processes in tomato .
	manualset3
226901	1	421145	7	NULL	NULL	0	NULL	Lymphoid cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphoid cells from immunized mice demonstrated increased MLTI responses to cells of the immunizing tumor but not to other PCT , indicating that the post-immunization MLTI responses were primarily to individual rather than shared tumor cell surface antigens .
	manualset3
226902	2	421145	7	NULL	NULL	0	NULL	immunized mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphoid cells from immunized mice demonstrated increased MLTI responses to cells of the immunizing tumor but not to other PCT , indicating that the post-immunization MLTI responses were primarily to individual rather than shared tumor cell surface antigens .
	manualset3
226903	3	421145	7	NULL	NULL	0	NULL	increased MLTI responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphoid cells from immunized mice demonstrated increased MLTI responses to cells of the immunizing tumor but not to other PCT , indicating that the post-immunization MLTI responses were primarily to individual rather than shared tumor cell surface antigens .
	manualset3
226904	4	421145	7	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphoid cells from immunized mice demonstrated increased MLTI responses to cells of the immunizing tumor but not to other PCT , indicating that the post-immunization MLTI responses were primarily to individual rather than shared tumor cell surface antigens .
	manualset3
226905	5	421145	7	NULL	NULL	0	NULL	immunizing tumor	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphoid cells from immunized mice demonstrated increased MLTI responses to cells of the immunizing tumor but not to other PCT , indicating that the post-immunization MLTI responses were primarily to individual rather than shared tumor cell surface antigens .
	manualset3
226906	6	421145	7	NULL	NULL	0	NULL	 PCT	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphoid cells from immunized mice demonstrated increased MLTI responses to cells of the immunizing tumor but not to other PCT , indicating that the post-immunization MLTI responses were primarily to individual rather than shared tumor cell surface antigens .
	manualset3
226907	7	421145	7	NULL	NULL	0	NULL	post-immunization MLTI responses 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphoid cells from immunized mice demonstrated increased MLTI responses to cells of the immunizing tumor but not to other PCT , indicating that the post-immunization MLTI responses were primarily to individual rather than shared tumor cell surface antigens .
	manualset3
226908	9	421145	7	NULL	NULL	NULL	NULL	 shared tumor cell surface antigens	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Lymphoid cells from immunized mice demonstrated increased MLTI responses to cells of the immunizing tumor but not to other PCT , indicating that the post-immunization MLTI responses were primarily to individual rather than shared tumor cell surface antigens .
	manualset3
226909	8	421145	7	NULL	NULL	0	NULL	individual	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Lymphoid cells from immunized mice demonstrated increased MLTI responses to cells of the immunizing tumor but not to other PCT , indicating that the post-immunization MLTI responses were primarily to individual rather than shared tumor cell surface antigens .
	manualset3
226910	1	421146	7	NULL	NULL	0	NULL	initial cytologic diagnoses 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial cytologic diagnoses were 10 carcinomas , eight suspicious for carcinoma , and two cases were misinterpreted as fibroadenoma .
	manualset3
226911	2	421146	7	NULL	NULL	0	NULL	10 carcinomas 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial cytologic diagnoses were 10 carcinomas , eight suspicious for carcinoma , and two cases were misinterpreted as fibroadenoma .
	manualset3
226912	3	421146	7	NULL	NULL	0	NULL	eight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial cytologic diagnoses were 10 carcinomas , eight suspicious for carcinoma , and two cases were misinterpreted as fibroadenoma .
	manualset3
226913	4	421146	7	NULL	NULL	0	NULL	carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial cytologic diagnoses were 10 carcinomas , eight suspicious for carcinoma , and two cases were misinterpreted as fibroadenoma .
	manualset3
226914	5	421146	7	NULL	NULL	0	NULL	two cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial cytologic diagnoses were 10 carcinomas , eight suspicious for carcinoma , and two cases were misinterpreted as fibroadenoma .
	manualset3
226915	6	421146	7	NULL	NULL	0	NULL	fibroadenoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The initial cytologic diagnoses were 10 carcinomas , eight suspicious for carcinoma , and two cases were misinterpreted as fibroadenoma .
	manualset3
226916	1	421147	7	NULL	NULL	0	NULL	antihypertensive medication 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Among those who did not report taking antihypertensive medication in midlife , 27 % ( 95 % CI : 8.9 % to 42.1 % ) of dementia cases can be attributed to systolic BP ) or = 120 mm Hg , translating into 17 excess cases per 1000 .
	manualset3
226917	2	421147	7	NULL	NULL	0	NULL	midlife	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Among those who did not report taking antihypertensive medication in midlife , 27 % ( 95 % CI : 8.9 % to 42.1 % ) of dementia cases can be attributed to systolic BP ) or = 120 mm Hg , translating into 17 excess cases per 1000 .
	manualset3
226918	3	421147	7	NULL	NULL	0	NULL	27 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among those who did not report taking antihypertensive medication in midlife , 27 % ( 95 % CI : 8.9 % to 42.1 % ) of dementia cases can be attributed to systolic BP ) or = 120 mm Hg , translating into 17 excess cases per 1000 .
	manualset3
226919	4	421147	7	NULL	NULL	NULL	NULL	95 % CI	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Among those who did not report taking antihypertensive medication in midlife , 27 % ( 95 % CI : 8.9 % to 42.1 % ) of dementia cases can be attributed to systolic BP ) or = 120 mm Hg , translating into 17 excess cases per 1000 .
	manualset3
226920	5	421147	7	NULL	NULL	0	NULL	8.9 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among those who did not report taking antihypertensive medication in midlife , 27 % ( 95 % CI : 8.9 % to 42.1 % ) of dementia cases can be attributed to systolic BP ) or = 120 mm Hg , translating into 17 excess cases per 1000 .
	manualset3
226921	6	421147	7	NULL	NULL	0	NULL	42.1 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among those who did not report taking antihypertensive medication in midlife , 27 % ( 95 % CI : 8.9 % to 42.1 % ) of dementia cases can be attributed to systolic BP ) or = 120 mm Hg , translating into 17 excess cases per 1000 .
	manualset3
226922	7	421147	7	NULL	NULL	0	NULL	dementia cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among those who did not report taking antihypertensive medication in midlife , 27 % ( 95 % CI : 8.9 % to 42.1 % ) of dementia cases can be attributed to systolic BP ) or = 120 mm Hg , translating into 17 excess cases per 1000 .
	manualset3
226923	8	421147	7	NULL	NULL	0	NULL	systolic BP	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among those who did not report taking antihypertensive medication in midlife , 27 % ( 95 % CI : 8.9 % to 42.1 % ) of dementia cases can be attributed to systolic BP ) or = 120 mm Hg , translating into 17 excess cases per 1000 .
	manualset3
226924	9	421147	7	NULL	NULL	0	NULL	120 mm Hg	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among those who did not report taking antihypertensive medication in midlife , 27 % ( 95 % CI : 8.9 % to 42.1 % ) of dementia cases can be attributed to systolic BP ) or = 120 mm Hg , translating into 17 excess cases per 1000 .
	manualset3
226925	10	421147	7	NULL	NULL	0	NULL	17 excess cases per 1000	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among those who did not report taking antihypertensive medication in midlife , 27 % ( 95 % CI : 8.9 % to 42.1 % ) of dementia cases can be attributed to systolic BP ) or = 120 mm Hg , translating into 17 excess cases per 1000 .
	manualset3
226926	1	421148	7	NULL	NULL	0	NULL	contribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The Contribution of Notch Signaling to Glioblastoma via Activation of Cancer Stem Cell Self-renewal : The Role of the Endothelial Network .
	manualset3
226927	2	421148	7	NULL	NULL	0	NULL	Notch Signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Contribution of Notch Signaling to Glioblastoma via Activation of Cancer Stem Cell Self-renewal : The Role of the Endothelial Network .
	manualset3
226928	3	421148	7	NULL	NULL	0	NULL	 Glioblastoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The Contribution of Notch Signaling to Glioblastoma via Activation of Cancer Stem Cell Self-renewal : The Role of the Endothelial Network .
	manualset3
226929	4	421148	7	NULL	NULL	NULL	NULL	Activation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The Contribution of Notch Signaling to Glioblastoma via Activation of Cancer Stem Cell Self-renewal : The Role of the Endothelial Network .
	manualset3
226930	5	421148	7	NULL	NULL	0	NULL	Cancer Stem Cell Self-renewal	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Contribution of Notch Signaling to Glioblastoma via Activation of Cancer Stem Cell Self-renewal : The Role of the Endothelial Network .
	manualset3
226931	6	421148	7	NULL	NULL	0	NULL	Role 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Contribution of Notch Signaling to Glioblastoma via Activation of Cancer Stem Cell Self-renewal : The Role of the Endothelial Network .
	manualset3
226932	7	421148	7	NULL	NULL	0	NULL	Endothelial Network	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The Contribution of Notch Signaling to Glioblastoma via Activation of Cancer Stem Cell Self-renewal : The Role of the Endothelial Network .
	manualset3
226933	1	421149	7	NULL	NULL	0	NULL	Occurrence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence and association of amyloid with diseases in birds and mammals including man : A review .
	manualset3
226934	2	421149	7	NULL	NULL	0	NULL	association 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence and association of amyloid with diseases in birds and mammals including man : A review .
	manualset3
226935	3	421149	7	NULL	NULL	0	NULL	amyloid	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence and association of amyloid with diseases in birds and mammals including man : A review .
	manualset3
226936	4	421149	7	NULL	NULL	0	NULL	diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence and association of amyloid with diseases in birds and mammals including man : A review .
	manualset3
226937	5	421149	7	NULL	NULL	0	NULL	birds	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence and association of amyloid with diseases in birds and mammals including man : A review .
	manualset3
226938	6	421149	7	NULL	NULL	0	NULL	mammals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence and association of amyloid with diseases in birds and mammals including man : A review .
	manualset3
226939	7	421149	7	NULL	NULL	0	NULL	man	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence and association of amyloid with diseases in birds and mammals including man : A review .
	manualset3
226940	8	421149	7	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Occurrence and association of amyloid with diseases in birds and mammals including man : A review .
	manualset3
226941	1	421150	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The relation of germ cells per tubule in testes , serum inhibin B and FSH in cryptorchid boys .
	manualset3
226942	2	421150	7	NULL	NULL	0	NULL	 germ cells per tubule	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The relation of germ cells per tubule in testes , serum inhibin B and FSH in cryptorchid boys .
	manualset3
226943	3	421150	7	NULL	NULL	0	NULL	testes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The relation of germ cells per tubule in testes , serum inhibin B and FSH in cryptorchid boys .
	manualset3
226944	4	421150	7	NULL	NULL	0	NULL	serum inhibin B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The relation of germ cells per tubule in testes , serum inhibin B and FSH in cryptorchid boys .
	manualset3
226945	5	421150	7	NULL	NULL	0	NULL	FSH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The relation of germ cells per tubule in testes , serum inhibin B and FSH in cryptorchid boys .
	manualset3
226946	6	421150	7	NULL	NULL	0	NULL	cryptorchid boys	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The relation of germ cells per tubule in testes , serum inhibin B and FSH in cryptorchid boys .
	manualset3
226947	1	421151	7	NULL	NULL	0	NULL	Definitive therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Definitive therapy consisted of laser coagulation of the valves and transient percutaneous drainage of the cysts .
	manualset3
226948	2	421151	7	NULL	NULL	0	NULL	laser coagulation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Definitive therapy consisted of laser coagulation of the valves and transient percutaneous drainage of the cysts .
	manualset3
226949	3	421151	7	NULL	NULL	0	NULL	valves	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Definitive therapy consisted of laser coagulation of the valves and transient percutaneous drainage of the cysts .
	manualset3
226950	4	421151	7	NULL	NULL	0	NULL	transient percutaneous drainage	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Definitive therapy consisted of laser coagulation of the valves and transient percutaneous drainage of the cysts .
	manualset3
226951	5	421151	7	NULL	NULL	0	NULL	 cysts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Definitive therapy consisted of laser coagulation of the valves and transient percutaneous drainage of the cysts .
	manualset3
226952	1	421152	7	NULL	NULL	0	NULL	Cloning	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Cloning and functional expression of alternative spliced variants of the human metabotropic glutamate receptor 8 .
	manualset3
226953	2	421152	7	NULL	NULL	0	NULL	functional expression	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Cloning and functional expression of alternative spliced variants of the human metabotropic glutamate receptor 8 .
	manualset3
226954	3	421152	7	NULL	NULL	NULL	NULL	 alternative spliced variants	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cloning and functional expression of alternative spliced variants of the human metabotropic glutamate receptor 8 .
	manualset3
226955	4	421152	7	NULL	NULL	0	NULL	human metabotropic glutamate receptor 8	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Cloning and functional expression of alternative spliced variants of the human metabotropic glutamate receptor 8 .
	manualset3
226956	1	421153	7	NULL	NULL	0	NULL	new formation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although a new formation of local recurrences can not be excluded for the further observation time and despite the small number of patients , the rate of recurrence-free patients suffering from tumors of stage T3N + signifies a most promising therapeutic approach .
	manualset3
226957	2	421153	7	NULL	NULL	0	NULL	local recurrences	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although a new formation of local recurrences can not be excluded for the further observation time and despite the small number of patients , the rate of recurrence-free patients suffering from tumors of stage T3N + signifies a most promising therapeutic approach .
	manualset3
226958	3	421153	7	NULL	NULL	0	NULL	observation time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Although a new formation of local recurrences can not be excluded for the further observation time and despite the small number of patients , the rate of recurrence-free patients suffering from tumors of stage T3N + signifies a most promising therapeutic approach .
	manualset3
226959	4	421153	7	NULL	NULL	0	NULL	small number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although a new formation of local recurrences can not be excluded for the further observation time and despite the small number of patients , the rate of recurrence-free patients suffering from tumors of stage T3N + signifies a most promising therapeutic approach .
	manualset3
226960	5	421153	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although a new formation of local recurrences can not be excluded for the further observation time and despite the small number of patients , the rate of recurrence-free patients suffering from tumors of stage T3N + signifies a most promising therapeutic approach .
	manualset3
226961	6	421153	7	NULL	NULL	0	NULL	rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although a new formation of local recurrences can not be excluded for the further observation time and despite the small number of patients , the rate of recurrence-free patients suffering from tumors of stage T3N + signifies a most promising therapeutic approach .
	manualset3
226962	7	421153	7	NULL	NULL	0	NULL	recurrence-free patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although a new formation of local recurrences can not be excluded for the further observation time and despite the small number of patients , the rate of recurrence-free patients suffering from tumors of stage T3N + signifies a most promising therapeutic approach .
	manualset3
226963	8	421153	7	NULL	NULL	0	NULL	tumors 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Although a new formation of local recurrences can not be excluded for the further observation time and despite the small number of patients , the rate of recurrence-free patients suffering from tumors of stage T3N + signifies a most promising therapeutic approach .
	manualset3
226964	9	421153	7	NULL	NULL	0	NULL	T3N +	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although a new formation of local recurrences can not be excluded for the further observation time and despite the small number of patients , the rate of recurrence-free patients suffering from tumors of stage T3N + signifies a most promising therapeutic approach .
	manualset3
226965	10	421153	7	NULL	NULL	0	NULL	therapeutic approach	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Although a new formation of local recurrences can not be excluded for the further observation time and despite the small number of patients , the rate of recurrence-free patients suffering from tumors of stage T3N + signifies a most promising therapeutic approach .
	manualset3
226966	1	421154	7	NULL	NULL	0	NULL	whites 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among whites , however , the prevalence of current smokers was slightly higher , and of heavy smokers was significantly higher , than national rates for whites ; while among blacks , smoking prevalence and amount were below national rates for blacks .
	manualset3
226967	2	421154	7	NULL	NULL	0	NULL	prevalence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among whites , however , the prevalence of current smokers was slightly higher , and of heavy smokers was significantly higher , than national rates for whites ; while among blacks , smoking prevalence and amount were below national rates for blacks .
	manualset3
226968	3	421154	7	NULL	NULL	0	NULL	current smokers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among whites , however , the prevalence of current smokers was slightly higher , and of heavy smokers was significantly higher , than national rates for whites ; while among blacks , smoking prevalence and amount were below national rates for blacks .
	manualset3
226969	4	421154	7	NULL	NULL	0	NULL	heavy smokers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among whites , however , the prevalence of current smokers was slightly higher , and of heavy smokers was significantly higher , than national rates for whites ; while among blacks , smoking prevalence and amount were below national rates for blacks .
	manualset3
226970	5	421154	7	NULL	NULL	0	NULL	national rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among whites , however , the prevalence of current smokers was slightly higher , and of heavy smokers was significantly higher , than national rates for whites ; while among blacks , smoking prevalence and amount were below national rates for blacks .
	manualset3
226971	6	421154	7	NULL	NULL	0	NULL	whites	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among whites , however , the prevalence of current smokers was slightly higher , and of heavy smokers was significantly higher , than national rates for whites ; while among blacks , smoking prevalence and amount were below national rates for blacks .
	manualset3
226972	7	421154	7	NULL	NULL	0	NULL	blacks	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among whites , however , the prevalence of current smokers was slightly higher , and of heavy smokers was significantly higher , than national rates for whites ; while among blacks , smoking prevalence and amount were below national rates for blacks .
	manualset3
226973	8	421154	7	NULL	NULL	0	NULL	smoking prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among whites , however , the prevalence of current smokers was slightly higher , and of heavy smokers was significantly higher , than national rates for whites ; while among blacks , smoking prevalence and amount were below national rates for blacks .
	manualset3
226974	9	421154	7	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among whites , however , the prevalence of current smokers was slightly higher , and of heavy smokers was significantly higher , than national rates for whites ; while among blacks , smoking prevalence and amount were below national rates for blacks .
	manualset3
226975	10	421154	7	NULL	NULL	0	NULL	 national rates 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among whites , however , the prevalence of current smokers was slightly higher , and of heavy smokers was significantly higher , than national rates for whites ; while among blacks , smoking prevalence and amount were below national rates for blacks .
	manualset3
226976	11	421154	7	NULL	NULL	0	NULL	blacks	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among whites , however , the prevalence of current smokers was slightly higher , and of heavy smokers was significantly higher , than national rates for whites ; while among blacks , smoking prevalence and amount were below national rates for blacks .
	manualset3
226977	1	421155	7	NULL	NULL	0	NULL	ultrastructural findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The ultrastructural findings suggested a diagnosis of a partially differentiated Sertoli cell tumor .
	manualset3
226978	2	421155	7	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The ultrastructural findings suggested a diagnosis of a partially differentiated Sertoli cell tumor .
	manualset3
226979	3	421155	7	NULL	NULL	0	NULL	partially differentiated Sertoli cell tumor	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The ultrastructural findings suggested a diagnosis of a partially differentiated Sertoli cell tumor .
	manualset3
226980	1	421156	7	NULL	NULL	0	NULL	 Genetic structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Genetic structure of the Orlov trotter and the Russian trotter ) .
	manualset3
226981	2	421156	7	NULL	NULL	0	NULL	Orlov trotter	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Genetic structure of the Orlov trotter and the Russian trotter ) .
	manualset3
226982	3	421156	7	NULL	NULL	0	NULL	Russian trotter	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Genetic structure of the Orlov trotter and the Russian trotter ) .
	manualset3
226983	1	421157	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A study was done to determine the major antigenic factors of Bordetella pertussis strains isolated throughout Canada and whether these isolates have the same antigenic structure as the bacilli in the currently used vaccines .
	manualset3
226984	2	421157	7	NULL	NULL	0	NULL	major antigenic factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A study was done to determine the major antigenic factors of Bordetella pertussis strains isolated throughout Canada and whether these isolates have the same antigenic structure as the bacilli in the currently used vaccines .
	manualset3
226985	3	421157	7	NULL	NULL	0	NULL	Bordetella pertussis strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A study was done to determine the major antigenic factors of Bordetella pertussis strains isolated throughout Canada and whether these isolates have the same antigenic structure as the bacilli in the currently used vaccines .
	manualset3
226986	4	421157	7	NULL	NULL	0	NULL	Canada	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	A study was done to determine the major antigenic factors of Bordetella pertussis strains isolated throughout Canada and whether these isolates have the same antigenic structure as the bacilli in the currently used vaccines .
	manualset3
226987	5	421157	7	NULL	NULL	0	NULL	isolates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A study was done to determine the major antigenic factors of Bordetella pertussis strains isolated throughout Canada and whether these isolates have the same antigenic structure as the bacilli in the currently used vaccines .
	manualset3
226988	6	421157	7	NULL	NULL	0	NULL	antigenic structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A study was done to determine the major antigenic factors of Bordetella pertussis strains isolated throughout Canada and whether these isolates have the same antigenic structure as the bacilli in the currently used vaccines .
	manualset3
226989	7	421157	7	NULL	NULL	0	NULL	bacilli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A study was done to determine the major antigenic factors of Bordetella pertussis strains isolated throughout Canada and whether these isolates have the same antigenic structure as the bacilli in the currently used vaccines .
	manualset3
226990	8	421157	7	NULL	NULL	0	NULL	vaccines	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A study was done to determine the major antigenic factors of Bordetella pertussis strains isolated throughout Canada and whether these isolates have the same antigenic structure as the bacilli in the currently used vaccines .
	manualset3
226991	1	421158	7	NULL	NULL	0	NULL	 Prevention 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Prevention of perinatal mortality ) .
	manualset3
226992	2	421158	7	NULL	NULL	0	NULL	 perinatal mortality 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Prevention of perinatal mortality ) .
	manualset3
226993	1	421159	7	NULL	NULL	0	NULL	putative BH3 ( BCL2 homology 3 ) domain 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	We identified a putative BH3 ( BCL2 homology 3 ) domain within this N-terminal CRK fragment , which sensitizes isolated mitochondria to cytochrome c release and when mutated significantly reduces the apoptotic activity of CRK in vivo .
	manualset3
226994	2	421159	7	NULL	NULL	0	NULL	N-terminal CRK fragment	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	We identified a putative BH3 ( BCL2 homology 3 ) domain within this N-terminal CRK fragment , which sensitizes isolated mitochondria to cytochrome c release and when mutated significantly reduces the apoptotic activity of CRK in vivo .
	manualset3
226995	3	421159	7	NULL	NULL	0	NULL	 isolated mitochondria 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	We identified a putative BH3 ( BCL2 homology 3 ) domain within this N-terminal CRK fragment , which sensitizes isolated mitochondria to cytochrome c release and when mutated significantly reduces the apoptotic activity of CRK in vivo .
	manualset3
226996	4	421159	7	NULL	NULL	0	NULL	cytochrome c release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We identified a putative BH3 ( BCL2 homology 3 ) domain within this N-terminal CRK fragment , which sensitizes isolated mitochondria to cytochrome c release and when mutated significantly reduces the apoptotic activity of CRK in vivo .
	manualset3
226997	5	421159	7	NULL	NULL	0	NULL	apoptotic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We identified a putative BH3 ( BCL2 homology 3 ) domain within this N-terminal CRK fragment , which sensitizes isolated mitochondria to cytochrome c release and when mutated significantly reduces the apoptotic activity of CRK in vivo .
	manualset3
226998	6	421159	7	NULL	NULL	0	NULL	CRK 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We identified a putative BH3 ( BCL2 homology 3 ) domain within this N-terminal CRK fragment , which sensitizes isolated mitochondria to cytochrome c release and when mutated significantly reduces the apoptotic activity of CRK in vivo .
	manualset3
226999	1	421160	7	NULL	NULL	0	NULL	Cocaine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Cocaine as an abortive agent in cluster headache .
	manualset3
227000	2	421160	7	NULL	NULL	0	NULL	abortive agent 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Cocaine as an abortive agent in cluster headache .
	manualset3
227001	3	421160	7	NULL	NULL	0	NULL	cluster headache	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Cocaine as an abortive agent in cluster headache .
	manualset3
227002	1	421161	7	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the number of megakaryocytic colony forming units ( CFU-Mks ) was significantly reduced , particularly in the spleen .
	manualset3
227003	2	421161	7	NULL	NULL	0	NULL	megakaryocytic colony forming units ( CFU-Mks )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the number of megakaryocytic colony forming units ( CFU-Mks ) was significantly reduced , particularly in the spleen .
	manualset3
227004	3	421161	7	NULL	NULL	0	NULL	spleen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , the number of megakaryocytic colony forming units ( CFU-Mks ) was significantly reduced , particularly in the spleen .
	manualset3
227005	1	421162	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among women , the odds ratio for possible or definite exposure was 18.8 ( 95 % CI 4.1-86 .2 ) .
	manualset3
227006	2	421162	7	NULL	NULL	0	NULL	odds ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among women , the odds ratio for possible or definite exposure was 18.8 ( 95 % CI 4.1-86 .2 ) .
	manualset3
227007	3	421162	7	NULL	NULL	0	NULL	18.8 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Among women , the odds ratio for possible or definite exposure was 18.8 ( 95 % CI 4.1-86 .2 ) .
	manualset3
227008	4	421162	7	NULL	NULL	0	NULL	95 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among women , the odds ratio for possible or definite exposure was 18.8 ( 95 % CI 4.1-86 .2 ) .
	manualset3
227009	5	421162	7	NULL	NULL	0	NULL	CI 4.1-86 .2	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among women , the odds ratio for possible or definite exposure was 18.8 ( 95 % CI 4.1-86 .2 ) .
	manualset3
228686	6	421162	7	NULL	NULL	0	NULL	definite exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among women , the odds ratio for possible or definite exposure was 18.8 ( 95 % CI 4.1-86 .2 ) .
	manualset3
227010	1	421163	7	NULL	NULL	0	NULL	E. chaffeensis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	E. chaffeensis and other tick-transmitted pathogens have adapted to both the tick and vertebrate host cell environments .
	manualset3
227011	2	421163	7	NULL	NULL	0	NULL	tick-transmitted pathogens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	E. chaffeensis and other tick-transmitted pathogens have adapted to both the tick and vertebrate host cell environments .
	manualset3
227012	3	421163	7	NULL	NULL	0	NULL	tick	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	E. chaffeensis and other tick-transmitted pathogens have adapted to both the tick and vertebrate host cell environments .
	manualset3
227013	4	421163	7	NULL	NULL	0	NULL	vertebrate host cell environments	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	E. chaffeensis and other tick-transmitted pathogens have adapted to both the tick and vertebrate host cell environments .
	manualset3
227014	1	421164	7	NULL	NULL	0	NULL	short form	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a short form of the CPS and mixed models incorporating fixed and random effects , we examined the reliability , individual stability , mean-level stability , and predictive utility of juvenile psychopathy as a function of age ( i.e. , from 7 to 17 years old ) in over 1 , 500 boys from the three cohorts of the Pittsburgh Youth Study .
	manualset3
227015	2	421164	7	NULL	NULL	0	NULL	CPS	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a short form of the CPS and mixed models incorporating fixed and random effects , we examined the reliability , individual stability , mean-level stability , and predictive utility of juvenile psychopathy as a function of age ( i.e. , from 7 to 17 years old ) in over 1 , 500 boys from the three cohorts of the Pittsburgh Youth Study .
	manualset3
227016	3	421164	7	NULL	NULL	0	NULL	mixed models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a short form of the CPS and mixed models incorporating fixed and random effects , we examined the reliability , individual stability , mean-level stability , and predictive utility of juvenile psychopathy as a function of age ( i.e. , from 7 to 17 years old ) in over 1 , 500 boys from the three cohorts of the Pittsburgh Youth Study .
	manualset3
227017	4	421164	7	NULL	NULL	0	NULL	fixed effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a short form of the CPS and mixed models incorporating fixed and random effects , we examined the reliability , individual stability , mean-level stability , and predictive utility of juvenile psychopathy as a function of age ( i.e. , from 7 to 17 years old ) in over 1 , 500 boys from the three cohorts of the Pittsburgh Youth Study .
	manualset3
227018	5	421164	7	NULL	NULL	0	NULL	random effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a short form of the CPS and mixed models incorporating fixed and random effects , we examined the reliability , individual stability , mean-level stability , and predictive utility of juvenile psychopathy as a function of age ( i.e. , from 7 to 17 years old ) in over 1 , 500 boys from the three cohorts of the Pittsburgh Youth Study .
	manualset3
227019	6	421164	7	NULL	NULL	0	NULL	reliability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a short form of the CPS and mixed models incorporating fixed and random effects , we examined the reliability , individual stability , mean-level stability , and predictive utility of juvenile psychopathy as a function of age ( i.e. , from 7 to 17 years old ) in over 1 , 500 boys from the three cohorts of the Pittsburgh Youth Study .
	manualset3
227020	7	421164	7	NULL	NULL	0	NULL	 individual stability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a short form of the CPS and mixed models incorporating fixed and random effects , we examined the reliability , individual stability , mean-level stability , and predictive utility of juvenile psychopathy as a function of age ( i.e. , from 7 to 17 years old ) in over 1 , 500 boys from the three cohorts of the Pittsburgh Youth Study .
	manualset3
227021	8	421164	7	NULL	NULL	0	NULL	mean-level stability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a short form of the CPS and mixed models incorporating fixed and random effects , we examined the reliability , individual stability , mean-level stability , and predictive utility of juvenile psychopathy as a function of age ( i.e. , from 7 to 17 years old ) in over 1 , 500 boys from the three cohorts of the Pittsburgh Youth Study .
	manualset3
227022	9	421164	7	NULL	NULL	0	NULL	predictive utility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a short form of the CPS and mixed models incorporating fixed and random effects , we examined the reliability , individual stability , mean-level stability , and predictive utility of juvenile psychopathy as a function of age ( i.e. , from 7 to 17 years old ) in over 1 , 500 boys from the three cohorts of the Pittsburgh Youth Study .
	manualset3
227023	10	421164	7	NULL	NULL	0	NULL	juvenile psychopathy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a short form of the CPS and mixed models incorporating fixed and random effects , we examined the reliability , individual stability , mean-level stability , and predictive utility of juvenile psychopathy as a function of age ( i.e. , from 7 to 17 years old ) in over 1 , 500 boys from the three cohorts of the Pittsburgh Youth Study .
	manualset3
227024	11	421164	7	NULL	NULL	0	NULL	 function 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a short form of the CPS and mixed models incorporating fixed and random effects , we examined the reliability , individual stability , mean-level stability , and predictive utility of juvenile psychopathy as a function of age ( i.e. , from 7 to 17 years old ) in over 1 , 500 boys from the three cohorts of the Pittsburgh Youth Study .
	manualset3
227025	12	421164	7	NULL	NULL	0	NULL	age	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a short form of the CPS and mixed models incorporating fixed and random effects , we examined the reliability , individual stability , mean-level stability , and predictive utility of juvenile psychopathy as a function of age ( i.e. , from 7 to 17 years old ) in over 1 , 500 boys from the three cohorts of the Pittsburgh Youth Study .
	manualset3
227026	13	421164	7	NULL	NULL	0	NULL	7 to 17 years old 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a short form of the CPS and mixed models incorporating fixed and random effects , we examined the reliability , individual stability , mean-level stability , and predictive utility of juvenile psychopathy as a function of age ( i.e. , from 7 to 17 years old ) in over 1 , 500 boys from the three cohorts of the Pittsburgh Youth Study .
	manualset3
227027	14	421164	7	NULL	NULL	0	NULL	1 , 500 boys	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a short form of the CPS and mixed models incorporating fixed and random effects , we examined the reliability , individual stability , mean-level stability , and predictive utility of juvenile psychopathy as a function of age ( i.e. , from 7 to 17 years old ) in over 1 , 500 boys from the three cohorts of the Pittsburgh Youth Study .
	manualset3
227028	15	421164	7	NULL	NULL	0	NULL	three cohorts	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a short form of the CPS and mixed models incorporating fixed and random effects , we examined the reliability , individual stability , mean-level stability , and predictive utility of juvenile psychopathy as a function of age ( i.e. , from 7 to 17 years old ) in over 1 , 500 boys from the three cohorts of the Pittsburgh Youth Study .
	manualset3
227029	16	421164	7	NULL	NULL	0	NULL	Pittsburgh Youth Study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a short form of the CPS and mixed models incorporating fixed and random effects , we examined the reliability , individual stability , mean-level stability , and predictive utility of juvenile psychopathy as a function of age ( i.e. , from 7 to 17 years old ) in over 1 , 500 boys from the three cohorts of the Pittsburgh Youth Study .
	manualset3
227030	1	421165	7	NULL	NULL	0	NULL	purpose	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this cephalometric study was to analyze the treatment and post-treatment craniofacial effects of a facemask ( FM ) combined with a bite block ( BB ) with specific regard to the sagittal pharyngeal dimensions in subjects with a Class III malocclusion when compared with an untreated Class III control group .
	manualset3
227031	2	421165	7	NULL	NULL	0	NULL	cephalometric study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this cephalometric study was to analyze the treatment and post-treatment craniofacial effects of a facemask ( FM ) combined with a bite block ( BB ) with specific regard to the sagittal pharyngeal dimensions in subjects with a Class III malocclusion when compared with an untreated Class III control group .
	manualset3
227032	3	421165	7	NULL	NULL	0	NULL	 treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this cephalometric study was to analyze the treatment and post-treatment craniofacial effects of a facemask ( FM ) combined with a bite block ( BB ) with specific regard to the sagittal pharyngeal dimensions in subjects with a Class III malocclusion when compared with an untreated Class III control group .
	manualset3
227033	4	421165	7	NULL	NULL	0	NULL	 post-treatment craniofacial effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this cephalometric study was to analyze the treatment and post-treatment craniofacial effects of a facemask ( FM ) combined with a bite block ( BB ) with specific regard to the sagittal pharyngeal dimensions in subjects with a Class III malocclusion when compared with an untreated Class III control group .
	manualset3
227034	5	421165	7	NULL	NULL	NULL	NULL	 facemask ( FM )	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose of this cephalometric study was to analyze the treatment and post-treatment craniofacial effects of a facemask ( FM ) combined with a bite block ( BB ) with specific regard to the sagittal pharyngeal dimensions in subjects with a Class III malocclusion when compared with an untreated Class III control group .
	manualset3
227035	6	421165	7	NULL	NULL	NULL	NULL	bite block ( BB )	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The purpose of this cephalometric study was to analyze the treatment and post-treatment craniofacial effects of a facemask ( FM ) combined with a bite block ( BB ) with specific regard to the sagittal pharyngeal dimensions in subjects with a Class III malocclusion when compared with an untreated Class III control group .
	manualset3
227036	7	421165	7	NULL	NULL	0	NULL	sagittal pharyngeal dimensions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this cephalometric study was to analyze the treatment and post-treatment craniofacial effects of a facemask ( FM ) combined with a bite block ( BB ) with specific regard to the sagittal pharyngeal dimensions in subjects with a Class III malocclusion when compared with an untreated Class III control group .
	manualset3
227037	8	421165	7	NULL	NULL	0	NULL	 subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this cephalometric study was to analyze the treatment and post-treatment craniofacial effects of a facemask ( FM ) combined with a bite block ( BB ) with specific regard to the sagittal pharyngeal dimensions in subjects with a Class III malocclusion when compared with an untreated Class III control group .
	manualset3
227038	9	421165	7	NULL	NULL	0	NULL	Class III malocclusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this cephalometric study was to analyze the treatment and post-treatment craniofacial effects of a facemask ( FM ) combined with a bite block ( BB ) with specific regard to the sagittal pharyngeal dimensions in subjects with a Class III malocclusion when compared with an untreated Class III control group .
	manualset3
227039	10	421165	7	NULL	NULL	0	NULL	untreated Class III control group 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this cephalometric study was to analyze the treatment and post-treatment craniofacial effects of a facemask ( FM ) combined with a bite block ( BB ) with specific regard to the sagittal pharyngeal dimensions in subjects with a Class III malocclusion when compared with an untreated Class III control group .
	manualset3
227040	1	421166	7	NULL	NULL	0	NULL	mouse L cell line ( mGHR1 .6 )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A mouse L cell line ( mGHR1 .6 ) , which expresses high levels of full-length mGHR , was established .
	manualset3
227041	2	421166	7	NULL	NULL	0	NULL	high levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A mouse L cell line ( mGHR1 .6 ) , which expresses high levels of full-length mGHR , was established .
	manualset3
227042	3	421166	7	NULL	NULL	0	NULL	full-length mGHR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A mouse L cell line ( mGHR1 .6 ) , which expresses high levels of full-length mGHR , was established .
	manualset3
227043	1	421167	7	NULL	NULL	0	NULL	 practical approach 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A practical approach to the treatment of acne vulgaris .
	manualset3
227044	2	421167	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A practical approach to the treatment of acne vulgaris .
	manualset3
227045	3	421167	7	NULL	NULL	0	NULL	acne vulgaris	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A practical approach to the treatment of acne vulgaris .
	manualset3
227046	1	421168	7	NULL	NULL	0	NULL	Observations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Observations on birth planning in China , 1977 .
	manualset3
227047	2	421168	7	NULL	NULL	0	NULL	birth planning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Observations on birth planning in China , 1977 .
	manualset3
227048	3	421168	7	NULL	NULL	0	NULL	China	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Observations on birth planning in China , 1977 .
	manualset3
227049	4	421168	7	NULL	NULL	0	NULL	1977	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Observations on birth planning in China , 1977 .
	manualset3
227051	1	421169	7	NULL	NULL	0	NULL	Chronic wasting disease ( CWD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic wasting disease ( CWD ) is a fatal spongiform encephalopathy that is efficiently transmitted among members of the mammalian family Cervidae , including deer , elk , and moose .
	manualset3
227052	2	421169	7	NULL	NULL	0	NULL	fatal spongiform encephalopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic wasting disease ( CWD ) is a fatal spongiform encephalopathy that is efficiently transmitted among members of the mammalian family Cervidae , including deer , elk , and moose .
	manualset3
227053	3	421169	7	NULL	NULL	0	NULL	members	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic wasting disease ( CWD ) is a fatal spongiform encephalopathy that is efficiently transmitted among members of the mammalian family Cervidae , including deer , elk , and moose .
	manualset3
227054	4	421169	7	NULL	NULL	0	NULL	mammalian family	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic wasting disease ( CWD ) is a fatal spongiform encephalopathy that is efficiently transmitted among members of the mammalian family Cervidae , including deer , elk , and moose .
	manualset3
227055	5	421169	7	NULL	NULL	0	NULL	Cervidae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic wasting disease ( CWD ) is a fatal spongiform encephalopathy that is efficiently transmitted among members of the mammalian family Cervidae , including deer , elk , and moose .
	manualset3
227056	6	421169	7	NULL	NULL	0	NULL	deer	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic wasting disease ( CWD ) is a fatal spongiform encephalopathy that is efficiently transmitted among members of the mammalian family Cervidae , including deer , elk , and moose .
	manualset3
227057	7	421169	7	NULL	NULL	0	NULL	 elk	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic wasting disease ( CWD ) is a fatal spongiform encephalopathy that is efficiently transmitted among members of the mammalian family Cervidae , including deer , elk , and moose .
	manualset3
227058	8	421169	7	NULL	NULL	0	NULL	moose	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Chronic wasting disease ( CWD ) is a fatal spongiform encephalopathy that is efficiently transmitted among members of the mammalian family Cervidae , including deer , elk , and moose .
	manualset3
227059	1	421170	7	NULL	NULL	0	NULL	review 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with a review of the literature , we will define the risk factors , clinical characteristics , diagnostic methods , and treatment of actinomycosis .
	manualset3
227060	2	421170	7	NULL	NULL	0	NULL	literature 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with a review of the literature , we will define the risk factors , clinical characteristics , diagnostic methods , and treatment of actinomycosis .
	manualset3
227061	3	421170	7	NULL	NULL	0	NULL	risk factors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with a review of the literature , we will define the risk factors , clinical characteristics , diagnostic methods , and treatment of actinomycosis .
	manualset3
227062	4	421170	7	NULL	NULL	0	NULL	clinical characteristics	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with a review of the literature , we will define the risk factors , clinical characteristics , diagnostic methods , and treatment of actinomycosis .
	manualset3
227063	5	421170	7	NULL	NULL	0	NULL	diagnostic methods	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with a review of the literature , we will define the risk factors , clinical characteristics , diagnostic methods , and treatment of actinomycosis .
	manualset3
227064	6	421170	7	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with a review of the literature , we will define the risk factors , clinical characteristics , diagnostic methods , and treatment of actinomycosis .
	manualset3
227065	7	421170	7	NULL	NULL	0	NULL	actinomycosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Along with a review of the literature , we will define the risk factors , clinical characteristics , diagnostic methods , and treatment of actinomycosis .
	manualset3
227066	1	421171	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among women 13.3 % reported being pregnant , and among men 12.0 % reported their partner pregnant .
	manualset3
227067	2	421171	7	NULL	NULL	0	NULL	13.3 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among women 13.3 % reported being pregnant , and among men 12.0 % reported their partner pregnant .
	manualset3
227068	3	421171	7	NULL	NULL	0	NULL	pregnant	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among women 13.3 % reported being pregnant , and among men 12.0 % reported their partner pregnant .
	manualset3
227069	4	421171	7	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among women 13.3 % reported being pregnant , and among men 12.0 % reported their partner pregnant .
	manualset3
227070	5	421171	7	NULL	NULL	0	NULL	12.0 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among women 13.3 % reported being pregnant , and among men 12.0 % reported their partner pregnant .
	manualset3
227071	6	421171	7	NULL	NULL	NULL	NULL	partner 	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Among women 13.3 % reported being pregnant , and among men 12.0 % reported their partner pregnant .
	manualset3
227072	7	421171	7	NULL	NULL	0	NULL	pregnant	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among women 13.3 % reported being pregnant , and among men 12.0 % reported their partner pregnant .
	manualset3
227073	1	421172	7	NULL	NULL	0	NULL	Metabolism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Metabolism of lipid peroxides .
	manualset3
227074	2	421172	7	NULL	NULL	0	NULL	lipid peroxides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Metabolism of lipid peroxides .
	manualset3
227075	1	421173	7	NULL	NULL	0	NULL	Treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of DHF remains empirical and unsatisfactory because of the lack of large-scale randomized controlled trials in this area .
	manualset3
227076	2	421173	7	NULL	NULL	0	NULL	DHF 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of DHF remains empirical and unsatisfactory because of the lack of large-scale randomized controlled trials in this area .
	manualset3
227077	3	421173	7	NULL	NULL	0	NULL	 large-scale randomized controlled trials	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of DHF remains empirical and unsatisfactory because of the lack of large-scale randomized controlled trials in this area .
	manualset3
227078	4	421173	7	NULL	NULL	0	NULL	area	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of DHF remains empirical and unsatisfactory because of the lack of large-scale randomized controlled trials in this area .
	manualset3
227079	1	421174	7	NULL	NULL	0	NULL	PG levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The PG levels did not change significantly at any time from 03.00 to 08.00 h in group 1 but increased continuously from 6.7 + / - 0.5 mmol/l at 04.00 h to 7.8 + / - 0.5 mmol/l at 08.00 h ( P less than 0.01 ) in group 2 .
	manualset3
227080	2	421174	7	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The PG levels did not change significantly at any time from 03.00 to 08.00 h in group 1 but increased continuously from 6.7 + / - 0.5 mmol/l at 04.00 h to 7.8 + / - 0.5 mmol/l at 08.00 h ( P less than 0.01 ) in group 2 .
	manualset3
227081	3	421174	7	NULL	NULL	0	NULL	 03.00 to 08.00 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The PG levels did not change significantly at any time from 03.00 to 08.00 h in group 1 but increased continuously from 6.7 + / - 0.5 mmol/l at 04.00 h to 7.8 + / - 0.5 mmol/l at 08.00 h ( P less than 0.01 ) in group 2 .
	manualset3
227082	4	421174	7	NULL	NULL	0	NULL	group 1	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The PG levels did not change significantly at any time from 03.00 to 08.00 h in group 1 but increased continuously from 6.7 + / - 0.5 mmol/l at 04.00 h to 7.8 + / - 0.5 mmol/l at 08.00 h ( P less than 0.01 ) in group 2 .
	manualset3
227083	5	421174	7	NULL	NULL	0	NULL	6.7 + / - 0.5 mmol/l	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The PG levels did not change significantly at any time from 03.00 to 08.00 h in group 1 but increased continuously from 6.7 + / - 0.5 mmol/l at 04.00 h to 7.8 + / - 0.5 mmol/l at 08.00 h ( P less than 0.01 ) in group 2 .
	manualset3
227084	6	421174	7	NULL	NULL	0	NULL	 04.00 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The PG levels did not change significantly at any time from 03.00 to 08.00 h in group 1 but increased continuously from 6.7 + / - 0.5 mmol/l at 04.00 h to 7.8 + / - 0.5 mmol/l at 08.00 h ( P less than 0.01 ) in group 2 .
	manualset3
227085	7	421174	7	NULL	NULL	0	NULL	7.8 + / - 0.5 mmol/l	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The PG levels did not change significantly at any time from 03.00 to 08.00 h in group 1 but increased continuously from 6.7 + / - 0.5 mmol/l at 04.00 h to 7.8 + / - 0.5 mmol/l at 08.00 h ( P less than 0.01 ) in group 2 .
	manualset3
227086	8	421174	7	NULL	NULL	0	NULL	08.00 h	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The PG levels did not change significantly at any time from 03.00 to 08.00 h in group 1 but increased continuously from 6.7 + / - 0.5 mmol/l at 04.00 h to 7.8 + / - 0.5 mmol/l at 08.00 h ( P less than 0.01 ) in group 2 .
	manualset3
227087	9	421174	7	NULL	NULL	0	NULL	P less than 0.01	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The PG levels did not change significantly at any time from 03.00 to 08.00 h in group 1 but increased continuously from 6.7 + / - 0.5 mmol/l at 04.00 h to 7.8 + / - 0.5 mmol/l at 08.00 h ( P less than 0.01 ) in group 2 .
	manualset3
227088	10	421174	7	NULL	NULL	0	NULL	 group 2	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The PG levels did not change significantly at any time from 03.00 to 08.00 h in group 1 but increased continuously from 6.7 + / - 0.5 mmol/l at 04.00 h to 7.8 + / - 0.5 mmol/l at 08.00 h ( P less than 0.01 ) in group 2 .
	manualset3
227089	1	421175	7	NULL	NULL	0	NULL	Epidemiological evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiological evidence strongly suggests an association between cigarette smoking and pancreatic diseases .
	manualset3
227090	2	421175	7	NULL	NULL	0	NULL	association 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiological evidence strongly suggests an association between cigarette smoking and pancreatic diseases .
	manualset3
227091	3	421175	7	NULL	NULL	0	NULL	cigarette smoking	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiological evidence strongly suggests an association between cigarette smoking and pancreatic diseases .
	manualset3
227092	4	421175	7	NULL	NULL	0	NULL	pancreatic diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiological evidence strongly suggests an association between cigarette smoking and pancreatic diseases .
	manualset3
227093	1	421176	7	NULL	NULL	0	NULL	Glucocorticoids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Glucocorticoids exacerbate this hyperinsulinemic state , rendering an individual at further risk for chronic disease .
	manualset3
227094	2	421176	7	NULL	NULL	0	NULL	hyperinsulinemic state	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Glucocorticoids exacerbate this hyperinsulinemic state , rendering an individual at further risk for chronic disease .
	manualset3
227095	3	421176	7	NULL	NULL	0	NULL	individual 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Glucocorticoids exacerbate this hyperinsulinemic state , rendering an individual at further risk for chronic disease .
	manualset3
227096	4	421176	7	NULL	NULL	0	NULL	risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Glucocorticoids exacerbate this hyperinsulinemic state , rendering an individual at further risk for chronic disease .
	manualset3
227097	5	421176	7	NULL	NULL	0	NULL	chronic disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Glucocorticoids exacerbate this hyperinsulinemic state , rendering an individual at further risk for chronic disease .
	manualset3
227098	1	421177	7	NULL	NULL	0	NULL	model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A frequently used model is allergic contact dermatitis ( ACD ) ; however , this T-cell-mediated skin condition so far is not well characterized in pigs .
	manualset3
227099	2	421177	7	NULL	NULL	0	NULL	allergic contact dermatitis ( ACD ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A frequently used model is allergic contact dermatitis ( ACD ) ; however , this T-cell-mediated skin condition so far is not well characterized in pigs .
	manualset3
227100	3	421177	7	NULL	NULL	0	NULL	T-cell-mediated skin condition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A frequently used model is allergic contact dermatitis ( ACD ) ; however , this T-cell-mediated skin condition so far is not well characterized in pigs .
	manualset3
227101	4	421177	7	NULL	NULL	0	NULL	pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A frequently used model is allergic contact dermatitis ( ACD ) ; however , this T-cell-mediated skin condition so far is not well characterized in pigs .
	manualset3
227102	1	421178	7	NULL	NULL	0	NULL	Coronary artery aneurysm ( CAA ) formation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Coronary artery aneurysm ( CAA ) formation in the setting of an acute inflammatory state due to connective tissue disease is rare .
	manualset3
227103	2	421178	7	NULL	NULL	0	NULL	setting	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Coronary artery aneurysm ( CAA ) formation in the setting of an acute inflammatory state due to connective tissue disease is rare .
	manualset3
227104	3	421178	7	NULL	NULL	0	NULL	acute inflammatory state	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Coronary artery aneurysm ( CAA ) formation in the setting of an acute inflammatory state due to connective tissue disease is rare .
	manualset3
227105	4	421178	7	NULL	NULL	0	NULL	connective tissue disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Coronary artery aneurysm ( CAA ) formation in the setting of an acute inflammatory state due to connective tissue disease is rare .
	manualset3
227106	1	421179	7	NULL	NULL	0	NULL	oral self-administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , oral self-administration of ethanol at 0.27 + / - 0.02 g/kg over 20 min is not sufficient for stimulation of dopamine activity in the nucleus accumbens .
	manualset3
227107	2	421179	7	NULL	NULL	0	NULL	 ethanol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , oral self-administration of ethanol at 0.27 + / - 0.02 g/kg over 20 min is not sufficient for stimulation of dopamine activity in the nucleus accumbens .
	manualset3
227108	3	421179	7	NULL	NULL	0	NULL	0.27 + / - 0.02 g/kg	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , oral self-administration of ethanol at 0.27 + / - 0.02 g/kg over 20 min is not sufficient for stimulation of dopamine activity in the nucleus accumbens .
	manualset3
227109	4	421179	7	NULL	NULL	0	NULL	20 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , oral self-administration of ethanol at 0.27 + / - 0.02 g/kg over 20 min is not sufficient for stimulation of dopamine activity in the nucleus accumbens .
	manualset3
227110	5	421179	7	NULL	NULL	0	NULL	stimulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , oral self-administration of ethanol at 0.27 + / - 0.02 g/kg over 20 min is not sufficient for stimulation of dopamine activity in the nucleus accumbens .
	manualset3
227111	6	421179	7	NULL	NULL	0	NULL	dopamine activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , oral self-administration of ethanol at 0.27 + / - 0.02 g/kg over 20 min is not sufficient for stimulation of dopamine activity in the nucleus accumbens .
	manualset3
227112	7	421179	7	NULL	NULL	0	NULL	 nucleus accumbens	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , oral self-administration of ethanol at 0.27 + / - 0.02 g/kg over 20 min is not sufficient for stimulation of dopamine activity in the nucleus accumbens .
	manualset3
227113	1	421180	7	NULL	NULL	0	NULL	Tl-SPECT	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Tl-SPECT will be feasible for the evaluation of the effectiveness of the therapy for malignant brain tumors , because it reflects the effectiveness of the therapy earlier than CT or MRI .
	manualset3
227114	2	421180	7	NULL	NULL	0	NULL	evaluation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Tl-SPECT will be feasible for the evaluation of the effectiveness of the therapy for malignant brain tumors , because it reflects the effectiveness of the therapy earlier than CT or MRI .
	manualset3
227115	3	421180	7	NULL	NULL	0	NULL	effectiveness 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Tl-SPECT will be feasible for the evaluation of the effectiveness of the therapy for malignant brain tumors , because it reflects the effectiveness of the therapy earlier than CT or MRI .
	manualset3
227116	4	421180	7	NULL	NULL	0	NULL	 therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Tl-SPECT will be feasible for the evaluation of the effectiveness of the therapy for malignant brain tumors , because it reflects the effectiveness of the therapy earlier than CT or MRI .
	manualset3
227117	5	421180	7	NULL	NULL	0	NULL	malignant brain tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Tl-SPECT will be feasible for the evaluation of the effectiveness of the therapy for malignant brain tumors , because it reflects the effectiveness of the therapy earlier than CT or MRI .
	manualset3
227118	6	421180	7	NULL	NULL	0	NULL	effectiveness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Tl-SPECT will be feasible for the evaluation of the effectiveness of the therapy for malignant brain tumors , because it reflects the effectiveness of the therapy earlier than CT or MRI .
	manualset3
227119	7	421180	7	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Tl-SPECT will be feasible for the evaluation of the effectiveness of the therapy for malignant brain tumors , because it reflects the effectiveness of the therapy earlier than CT or MRI .
	manualset3
227120	8	421180	7	NULL	NULL	0	NULL	CT	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Tl-SPECT will be feasible for the evaluation of the effectiveness of the therapy for malignant brain tumors , because it reflects the effectiveness of the therapy earlier than CT or MRI .
	manualset3
227121	9	421180	7	NULL	NULL	0	NULL	MRI	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Tl-SPECT will be feasible for the evaluation of the effectiveness of the therapy for malignant brain tumors , because it reflects the effectiveness of the therapy earlier than CT or MRI .
	manualset3
227122	1	421181	7	NULL	NULL	0	NULL	Left ventricular hypertrophy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Left ventricular hypertrophy in hypertension .
	manualset3
227123	2	421181	7	NULL	NULL	0	NULL	hypertension	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Left ventricular hypertrophy in hypertension .
	manualset3
227124	1	421182	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results are in accord with other studies on sodium cholate which indicate that the self-association involves several species , and that it is not a monomer-n-mer self-association .
	manualset3
227125	2	421182	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results are in accord with other studies on sodium cholate which indicate that the self-association involves several species , and that it is not a monomer-n-mer self-association .
	manualset3
227126	3	421182	7	NULL	NULL	0	NULL	sodium cholate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results are in accord with other studies on sodium cholate which indicate that the self-association involves several species , and that it is not a monomer-n-mer self-association .
	manualset3
227127	4	421182	7	NULL	NULL	0	NULL	self-association	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results are in accord with other studies on sodium cholate which indicate that the self-association involves several species , and that it is not a monomer-n-mer self-association .
	manualset3
227128	5	421182	7	NULL	NULL	0	NULL	species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results are in accord with other studies on sodium cholate which indicate that the self-association involves several species , and that it is not a monomer-n-mer self-association .
	manualset3
227129	6	421182	7	NULL	NULL	0	NULL	monomer-n-mer self-association	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results are in accord with other studies on sodium cholate which indicate that the self-association involves several species , and that it is not a monomer-n-mer self-association .
	manualset3
227130	1	421183	7	NULL	NULL	0	NULL	 presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of a form of stretch reflex , previously described in the arm by other authors , has been confirmed in the gastrocnemius muscle of the human leg .
	manualset3
227131	2	421183	7	NULL	NULL	NULL	NULL	 form of stretch reflex	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The presence of a form of stretch reflex , previously described in the arm by other authors , has been confirmed in the gastrocnemius muscle of the human leg .
	manualset3
227132	3	421183	7	NULL	NULL	0	NULL	arm 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of a form of stretch reflex , previously described in the arm by other authors , has been confirmed in the gastrocnemius muscle of the human leg .
	manualset3
227133	4	421183	7	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of a form of stretch reflex , previously described in the arm by other authors , has been confirmed in the gastrocnemius muscle of the human leg .
	manualset3
227134	5	421183	7	NULL	NULL	0	NULL	gastrocnemius muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of a form of stretch reflex , previously described in the arm by other authors , has been confirmed in the gastrocnemius muscle of the human leg .
	manualset3
227135	6	421183	7	NULL	NULL	0	NULL	 human leg	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of a form of stretch reflex , previously described in the arm by other authors , has been confirmed in the gastrocnemius muscle of the human leg .
	manualset3
227136	1	421184	7	NULL	NULL	0	NULL	Lethality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lethality reached 5 % ( 9 cases ) , but always related to septicemia from S. aureus .
	manualset3
227137	2	421184	7	NULL	NULL	0	NULL	5 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Lethality reached 5 % ( 9 cases ) , but always related to septicemia from S. aureus .
	manualset3
227138	3	421184	7	NULL	NULL	0	NULL	9 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Lethality reached 5 % ( 9 cases ) , but always related to septicemia from S. aureus .
	manualset3
227139	4	421184	7	NULL	NULL	0	NULL	septicemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Lethality reached 5 % ( 9 cases ) , but always related to septicemia from S. aureus .
	manualset3
227140	5	421184	7	NULL	NULL	0	NULL	S. aureus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Lethality reached 5 % ( 9 cases ) , but always related to septicemia from S. aureus .
	manualset3
227141	1	421185	7	NULL	NULL	NULL	NULL	day	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A day in the life of a nurse : cardiac transplant nurse assists patient , family in dynamic process .
	manualset3
227142	2	421185	7	NULL	NULL	0	NULL	life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A day in the life of a nurse : cardiac transplant nurse assists patient , family in dynamic process .
	manualset3
227143	3	421185	7	NULL	NULL	0	NULL	nurse	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A day in the life of a nurse : cardiac transplant nurse assists patient , family in dynamic process .
	manualset3
227144	4	421185	7	NULL	NULL	0	NULL	cardiac transplant nurse	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A day in the life of a nurse : cardiac transplant nurse assists patient , family in dynamic process .
	manualset3
227145	5	421185	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A day in the life of a nurse : cardiac transplant nurse assists patient , family in dynamic process .
	manualset3
227146	6	421185	7	NULL	NULL	0	NULL	family	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	A day in the life of a nurse : cardiac transplant nurse assists patient , family in dynamic process .
	manualset3
227147	7	421185	7	NULL	NULL	NULL	NULL	dynamic process	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A day in the life of a nurse : cardiac transplant nurse assists patient , family in dynamic process .
	manualset3
227148	1	421186	7	NULL	NULL	0	NULL	greatest levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The greatest levels were found in the duodenum and jejunum , the principal sites for absorption , which were 2.5 - and 3-fold respectively above ileal levels .
	manualset3
227149	2	421186	7	NULL	NULL	0	NULL	duodenum 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The greatest levels were found in the duodenum and jejunum , the principal sites for absorption , which were 2.5 - and 3-fold respectively above ileal levels .
	manualset3
227150	3	421186	7	NULL	NULL	0	NULL	jejunum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The greatest levels were found in the duodenum and jejunum , the principal sites for absorption , which were 2.5 - and 3-fold respectively above ileal levels .
	manualset3
227151	4	421186	7	NULL	NULL	0	NULL	principal sites	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The greatest levels were found in the duodenum and jejunum , the principal sites for absorption , which were 2.5 - and 3-fold respectively above ileal levels .
	manualset3
227152	5	421186	7	NULL	NULL	0	NULL	absorption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The greatest levels were found in the duodenum and jejunum , the principal sites for absorption , which were 2.5 - and 3-fold respectively above ileal levels .
	manualset3
227153	6	421186	7	NULL	NULL	0	NULL	 2.5-fold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The greatest levels were found in the duodenum and jejunum , the principal sites for absorption , which were 2.5 - and 3-fold respectively above ileal levels .
	manualset3
227154	7	421186	7	NULL	NULL	0	NULL	3-fold 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The greatest levels were found in the duodenum and jejunum , the principal sites for absorption , which were 2.5 - and 3-fold respectively above ileal levels .
	manualset3
227155	8	421186	7	NULL	NULL	0	NULL	 ileal levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The greatest levels were found in the duodenum and jejunum , the principal sites for absorption , which were 2.5 - and 3-fold respectively above ileal levels .
	manualset3
227156	1	421187	7	NULL	NULL	0	NULL	four healthy men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In four healthy men treated with 5 microgram of the LRH agonist daily over 17 weeks basal FSH , LH , and testosterone levels decreased but spermatogenesis and potency were unaffected .
	manualset3
227157	2	421187	7	NULL	NULL	0	NULL	 5 microgram	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In four healthy men treated with 5 microgram of the LRH agonist daily over 17 weeks basal FSH , LH , and testosterone levels decreased but spermatogenesis and potency were unaffected .
	manualset3
227158	3	421187	7	NULL	NULL	0	NULL	LRH agonist	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In four healthy men treated with 5 microgram of the LRH agonist daily over 17 weeks basal FSH , LH , and testosterone levels decreased but spermatogenesis and potency were unaffected .
	manualset3
227159	4	421187	7	NULL	NULL	0	NULL	 daily	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In four healthy men treated with 5 microgram of the LRH agonist daily over 17 weeks basal FSH , LH , and testosterone levels decreased but spermatogenesis and potency were unaffected .
	manualset3
227160	5	421187	7	NULL	NULL	0	NULL	17 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In four healthy men treated with 5 microgram of the LRH agonist daily over 17 weeks basal FSH , LH , and testosterone levels decreased but spermatogenesis and potency were unaffected .
	manualset3
227161	6	421187	7	NULL	NULL	NULL	NULL	basal FSH levels	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In four healthy men treated with 5 microgram of the LRH agonist daily over 17 weeks basal FSH , LH , and testosterone levels decreased but spermatogenesis and potency were unaffected .
	manualset3
227162	7	421187	7	NULL	NULL	0	NULL	LH levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In four healthy men treated with 5 microgram of the LRH agonist daily over 17 weeks basal FSH , LH , and testosterone levels decreased but spermatogenesis and potency were unaffected .
	manualset3
227163	8	421187	7	NULL	NULL	0	NULL	testosterone levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In four healthy men treated with 5 microgram of the LRH agonist daily over 17 weeks basal FSH , LH , and testosterone levels decreased but spermatogenesis and potency were unaffected .
	manualset3
227164	9	421187	7	NULL	NULL	0	NULL	spermatogenesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In four healthy men treated with 5 microgram of the LRH agonist daily over 17 weeks basal FSH , LH , and testosterone levels decreased but spermatogenesis and potency were unaffected .
	manualset3
227165	1	421188	7	NULL	NULL	0	NULL	intact animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In intact animals this differential action on the arterial system may cause a long-term decrease in blood flow to relatively inactive tissues ( digestive and locomotory organs ) while increasing circulation to tissues involved in egg production ( ovotestis and oviduct ) .
	manualset3
227166	2	421188	7	NULL	NULL	0	NULL	differential action 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In intact animals this differential action on the arterial system may cause a long-term decrease in blood flow to relatively inactive tissues ( digestive and locomotory organs ) while increasing circulation to tissues involved in egg production ( ovotestis and oviduct ) .
	manualset3
227167	3	421188	7	NULL	NULL	0	NULL	arterial system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In intact animals this differential action on the arterial system may cause a long-term decrease in blood flow to relatively inactive tissues ( digestive and locomotory organs ) while increasing circulation to tissues involved in egg production ( ovotestis and oviduct ) .
	manualset3
227168	4	421188	7	NULL	NULL	NULL	NULL	 long-term decrease	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In intact animals this differential action on the arterial system may cause a long-term decrease in blood flow to relatively inactive tissues ( digestive and locomotory organs ) while increasing circulation to tissues involved in egg production ( ovotestis and oviduct ) .
	manualset3
227169	5	421188	7	NULL	NULL	0	NULL	blood flow	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In intact animals this differential action on the arterial system may cause a long-term decrease in blood flow to relatively inactive tissues ( digestive and locomotory organs ) while increasing circulation to tissues involved in egg production ( ovotestis and oviduct ) .
	manualset3
227170	6	421188	7	NULL	NULL	0	NULL	inactive tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In intact animals this differential action on the arterial system may cause a long-term decrease in blood flow to relatively inactive tissues ( digestive and locomotory organs ) while increasing circulation to tissues involved in egg production ( ovotestis and oviduct ) .
	manualset3
227171	7	421188	7	NULL	NULL	0	NULL	digestive organs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In intact animals this differential action on the arterial system may cause a long-term decrease in blood flow to relatively inactive tissues ( digestive and locomotory organs ) while increasing circulation to tissues involved in egg production ( ovotestis and oviduct ) .
	manualset3
227172	8	421188	7	NULL	NULL	0	NULL	 locomotory organs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In intact animals this differential action on the arterial system may cause a long-term decrease in blood flow to relatively inactive tissues ( digestive and locomotory organs ) while increasing circulation to tissues involved in egg production ( ovotestis and oviduct ) .
	manualset3
227173	9	421188	7	NULL	NULL	0	NULL	increasing circulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In intact animals this differential action on the arterial system may cause a long-term decrease in blood flow to relatively inactive tissues ( digestive and locomotory organs ) while increasing circulation to tissues involved in egg production ( ovotestis and oviduct ) .
	manualset3
227174	10	421188	7	NULL	NULL	0	NULL	tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In intact animals this differential action on the arterial system may cause a long-term decrease in blood flow to relatively inactive tissues ( digestive and locomotory organs ) while increasing circulation to tissues involved in egg production ( ovotestis and oviduct ) .
	manualset3
227175	11	421188	7	NULL	NULL	0	NULL	egg production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In intact animals this differential action on the arterial system may cause a long-term decrease in blood flow to relatively inactive tissues ( digestive and locomotory organs ) while increasing circulation to tissues involved in egg production ( ovotestis and oviduct ) .
	manualset3
227176	12	421188	7	NULL	NULL	0	NULL	ovotestis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In intact animals this differential action on the arterial system may cause a long-term decrease in blood flow to relatively inactive tissues ( digestive and locomotory organs ) while increasing circulation to tissues involved in egg production ( ovotestis and oviduct ) .
	manualset3
227177	13	421188	7	NULL	NULL	0	NULL	oviduct 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In intact animals this differential action on the arterial system may cause a long-term decrease in blood flow to relatively inactive tissues ( digestive and locomotory organs ) while increasing circulation to tissues involved in egg production ( ovotestis and oviduct ) .
	manualset3
227178	1	421189	7	NULL	NULL	0	NULL	membrane humidifier	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The membrane humidifier could produce good humidification .
	manualset3
227179	2	421189	7	NULL	NULL	0	NULL	 good humidification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The membrane humidifier could produce good humidification .
	manualset3
227180	1	421190	7	NULL	NULL	0	NULL	Hormone administration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Hormone administration resulted in 4.2-fold increase of luciferase activity in liver homogenates .
	manualset3
227181	2	421190	7	NULL	NULL	0	NULL	4.2-fold increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hormone administration resulted in 4.2-fold increase of luciferase activity in liver homogenates .
	manualset3
227182	3	421190	7	NULL	NULL	0	NULL	luciferase activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Hormone administration resulted in 4.2-fold increase of luciferase activity in liver homogenates .
	manualset3
227183	4	421190	7	NULL	NULL	0	NULL	liver homogenates	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Hormone administration resulted in 4.2-fold increase of luciferase activity in liver homogenates .
	manualset3
227184	1	421191	7	NULL	NULL	0	NULL	Pharmacologic chronotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacologic chronotherapy is a developing science that holds much hope for increasing the effectiveness of drug therapy and for reducing the incidence of toxic drug reactions .
	manualset3
227185	2	421191	7	NULL	NULL	0	NULL	developing science	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacologic chronotherapy is a developing science that holds much hope for increasing the effectiveness of drug therapy and for reducing the incidence of toxic drug reactions .
	manualset3
227187	4	421191	7	NULL	NULL	0	NULL	effectiveness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacologic chronotherapy is a developing science that holds much hope for increasing the effectiveness of drug therapy and for reducing the incidence of toxic drug reactions .
	manualset3
227188	5	421191	7	NULL	NULL	0	NULL	drug therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacologic chronotherapy is a developing science that holds much hope for increasing the effectiveness of drug therapy and for reducing the incidence of toxic drug reactions .
	manualset3
227189	6	421191	7	NULL	NULL	0	NULL	 incidence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacologic chronotherapy is a developing science that holds much hope for increasing the effectiveness of drug therapy and for reducing the incidence of toxic drug reactions .
	manualset3
227190	7	421191	7	NULL	NULL	NULL	NULL	toxic drug reactions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pharmacologic chronotherapy is a developing science that holds much hope for increasing the effectiveness of drug therapy and for reducing the incidence of toxic drug reactions .
	manualset3
233267	8	421191	7	NULL	NULL	0	NULL	hope	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacologic chronotherapy is a developing science that holds much hope for increasing the effectiveness of drug therapy and for reducing the incidence of toxic drug reactions .
	manualset3
227191	1	421192	7	NULL	NULL	0	NULL	Host response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Host response to myeloma : I. Induction of cytotoxic and suppressor T cells by in vivo immunization with MOPC 104E plasmacytoma .
	manualset3
227192	2	421192	7	NULL	NULL	0	NULL	myeloma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Host response to myeloma : I. Induction of cytotoxic and suppressor T cells by in vivo immunization with MOPC 104E plasmacytoma .
	manualset3
227193	3	421192	7	NULL	NULL	0	NULL	Induction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Host response to myeloma : I. Induction of cytotoxic and suppressor T cells by in vivo immunization with MOPC 104E plasmacytoma .
	manualset3
227194	4	421192	7	NULL	NULL	0	NULL	cytotoxic T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Host response to myeloma : I. Induction of cytotoxic and suppressor T cells by in vivo immunization with MOPC 104E plasmacytoma .
	manualset3
227195	5	421192	7	NULL	NULL	0	NULL	suppressor T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Host response to myeloma : I. Induction of cytotoxic and suppressor T cells by in vivo immunization with MOPC 104E plasmacytoma .
	manualset3
227196	6	421192	7	NULL	NULL	0	NULL	in vivo immunization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Host response to myeloma : I. Induction of cytotoxic and suppressor T cells by in vivo immunization with MOPC 104E plasmacytoma .
	manualset3
227197	7	421192	7	NULL	NULL	0	NULL	MOPC 104E plasmacytoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Host response to myeloma : I. Induction of cytotoxic and suppressor T cells by in vivo immunization with MOPC 104E plasmacytoma .
	manualset3
227198	1	421193	7	NULL	NULL	0	NULL	Amphipathic protein toxins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Amphipathic protein toxins from tarantula venom inhibit voltage-activated potassium ( Kv ) channels by binding to a critical helix-turn-helix motif termed the voltage sensor paddle .
	manualset3
227199	2	421193	7	NULL	NULL	0	NULL	tarantula venom	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Amphipathic protein toxins from tarantula venom inhibit voltage-activated potassium ( Kv ) channels by binding to a critical helix-turn-helix motif termed the voltage sensor paddle .
	manualset3
227200	3	421193	7	NULL	NULL	NULL	NULL	voltage-activated potassium ( Kv ) channels	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Amphipathic protein toxins from tarantula venom inhibit voltage-activated potassium ( Kv ) channels by binding to a critical helix-turn-helix motif termed the voltage sensor paddle .
	manualset3
227201	4	421193	7	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Amphipathic protein toxins from tarantula venom inhibit voltage-activated potassium ( Kv ) channels by binding to a critical helix-turn-helix motif termed the voltage sensor paddle .
	manualset3
227202	5	421193	7	NULL	NULL	0	NULL	helix-turn-helix motif 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Amphipathic protein toxins from tarantula venom inhibit voltage-activated potassium ( Kv ) channels by binding to a critical helix-turn-helix motif termed the voltage sensor paddle .
	manualset3
227203	6	421193	7	NULL	NULL	0	NULL	voltage sensor paddle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Amphipathic protein toxins from tarantula venom inhibit voltage-activated potassium ( Kv ) channels by binding to a critical helix-turn-helix motif termed the voltage sensor paddle .
	manualset3
227204	1	421194	7	NULL	NULL	0	NULL	SIH	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , SIH is initially managed by conservative treatment .
	manualset3
227205	2	421194	7	NULL	NULL	0	NULL	conservative treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Traditionally , SIH is initially managed by conservative treatment .
	manualset3
227206	1	421195	7	NULL	NULL	0	NULL	absence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably , the absence of both Myb and Mip130 , or of both Myb and E2F2 , caused variegated expression in which high or low levels of Polo were stably inherited through successive cell divisions in imaginal wing discs .
	manualset3
227207	2	421195	7	NULL	NULL	0	NULL	Myb	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably , the absence of both Myb and Mip130 , or of both Myb and E2F2 , caused variegated expression in which high or low levels of Polo were stably inherited through successive cell divisions in imaginal wing discs .
	manualset3
227208	3	421195	7	NULL	NULL	0	NULL	Mip130	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably , the absence of both Myb and Mip130 , or of both Myb and E2F2 , caused variegated expression in which high or low levels of Polo were stably inherited through successive cell divisions in imaginal wing discs .
	manualset3
227209	4	421195	7	NULL	NULL	0	NULL	 Myb	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably , the absence of both Myb and Mip130 , or of both Myb and E2F2 , caused variegated expression in which high or low levels of Polo were stably inherited through successive cell divisions in imaginal wing discs .
	manualset3
227210	5	421195	7	NULL	NULL	0	NULL	E2F2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably , the absence of both Myb and Mip130 , or of both Myb and E2F2 , caused variegated expression in which high or low levels of Polo were stably inherited through successive cell divisions in imaginal wing discs .
	manualset3
227211	6	421195	7	NULL	NULL	0	NULL	 variegated expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably , the absence of both Myb and Mip130 , or of both Myb and E2F2 , caused variegated expression in which high or low levels of Polo were stably inherited through successive cell divisions in imaginal wing discs .
	manualset3
227212	7	421195	7	NULL	NULL	0	NULL	high levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably , the absence of both Myb and Mip130 , or of both Myb and E2F2 , caused variegated expression in which high or low levels of Polo were stably inherited through successive cell divisions in imaginal wing discs .
	manualset3
227213	8	421195	7	NULL	NULL	0	NULL	Polo	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably , the absence of both Myb and Mip130 , or of both Myb and E2F2 , caused variegated expression in which high or low levels of Polo were stably inherited through successive cell divisions in imaginal wing discs .
	manualset3
227214	9	421195	7	NULL	NULL	0	NULL	successive cell divisions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably , the absence of both Myb and Mip130 , or of both Myb and E2F2 , caused variegated expression in which high or low levels of Polo were stably inherited through successive cell divisions in imaginal wing discs .
	manualset3
227215	10	421195	7	NULL	NULL	0	NULL	imaginal wing discs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably , the absence of both Myb and Mip130 , or of both Myb and E2F2 , caused variegated expression in which high or low levels of Polo were stably inherited through successive cell divisions in imaginal wing discs .
	manualset3
228706	11	421195	7	NULL	NULL	0	NULL	low levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably , the absence of both Myb and Mip130 , or of both Myb and E2F2 , caused variegated expression in which high or low levels of Polo were stably inherited through successive cell divisions in imaginal wing discs .
	manualset3
227216	1	421196	7	NULL	NULL	0	NULL	2 - ( 2 - ( 1 , 4-Benzodioxanyl ) ) -2 - imidazoline ( RX 781094 ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	2 - ( 2 - ( 1 , 4-Benzodioxanyl ) ) -2 - imidazoline ( RX 781094 ) 0.1 or 1 microM reduced the overflow of 3H-noradrenaline and total tritium elicited by 13 electrical pulses at 0.25 Hz or 26 Pulses at 0.5 Hz .
	manualset3
227217	2	421196	7	NULL	NULL	0	NULL	0.1 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	2 - ( 2 - ( 1 , 4-Benzodioxanyl ) ) -2 - imidazoline ( RX 781094 ) 0.1 or 1 microM reduced the overflow of 3H-noradrenaline and total tritium elicited by 13 electrical pulses at 0.25 Hz or 26 Pulses at 0.5 Hz .
	manualset3
227218	3	421196	7	NULL	NULL	0	NULL	1 microM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	2 - ( 2 - ( 1 , 4-Benzodioxanyl ) ) -2 - imidazoline ( RX 781094 ) 0.1 or 1 microM reduced the overflow of 3H-noradrenaline and total tritium elicited by 13 electrical pulses at 0.25 Hz or 26 Pulses at 0.5 Hz .
	manualset3
227219	4	421196	7	NULL	NULL	0	NULL	overflow	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	2 - ( 2 - ( 1 , 4-Benzodioxanyl ) ) -2 - imidazoline ( RX 781094 ) 0.1 or 1 microM reduced the overflow of 3H-noradrenaline and total tritium elicited by 13 electrical pulses at 0.25 Hz or 26 Pulses at 0.5 Hz .
	manualset3
227220	5	421196	7	NULL	NULL	0	NULL	3H-noradrenaline	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	2 - ( 2 - ( 1 , 4-Benzodioxanyl ) ) -2 - imidazoline ( RX 781094 ) 0.1 or 1 microM reduced the overflow of 3H-noradrenaline and total tritium elicited by 13 electrical pulses at 0.25 Hz or 26 Pulses at 0.5 Hz .
	manualset3
227221	6	421196	7	NULL	NULL	0	NULL	total tritium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	2 - ( 2 - ( 1 , 4-Benzodioxanyl ) ) -2 - imidazoline ( RX 781094 ) 0.1 or 1 microM reduced the overflow of 3H-noradrenaline and total tritium elicited by 13 electrical pulses at 0.25 Hz or 26 Pulses at 0.5 Hz .
	manualset3
227222	7	421196	7	NULL	NULL	0	NULL	13 electrical pulses	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	2 - ( 2 - ( 1 , 4-Benzodioxanyl ) ) -2 - imidazoline ( RX 781094 ) 0.1 or 1 microM reduced the overflow of 3H-noradrenaline and total tritium elicited by 13 electrical pulses at 0.25 Hz or 26 Pulses at 0.5 Hz .
	manualset3
227223	8	421196	7	NULL	NULL	0	NULL	 0.25 Hz 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	2 - ( 2 - ( 1 , 4-Benzodioxanyl ) ) -2 - imidazoline ( RX 781094 ) 0.1 or 1 microM reduced the overflow of 3H-noradrenaline and total tritium elicited by 13 electrical pulses at 0.25 Hz or 26 Pulses at 0.5 Hz .
	manualset3
227224	9	421196	7	NULL	NULL	0	NULL	26 Pulses	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	2 - ( 2 - ( 1 , 4-Benzodioxanyl ) ) -2 - imidazoline ( RX 781094 ) 0.1 or 1 microM reduced the overflow of 3H-noradrenaline and total tritium elicited by 13 electrical pulses at 0.25 Hz or 26 Pulses at 0.5 Hz .
	manualset3
227225	10	421196	7	NULL	NULL	0	NULL	0.5 Hz	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	2 - ( 2 - ( 1 , 4-Benzodioxanyl ) ) -2 - imidazoline ( RX 781094 ) 0.1 or 1 microM reduced the overflow of 3H-noradrenaline and total tritium elicited by 13 electrical pulses at 0.25 Hz or 26 Pulses at 0.5 Hz .
	manualset3
227226	1	421197	7	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Despite these differences , second-derivative analysis of the v1 , v3 regions revealed no significant changes in the positions of the underlying bands used to characterize the environments of the phosphate ion in poorly crystalline HA .
	manualset3
227227	2	421197	7	NULL	NULL	0	NULL	second-derivative analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Despite these differences , second-derivative analysis of the v1 , v3 regions revealed no significant changes in the positions of the underlying bands used to characterize the environments of the phosphate ion in poorly crystalline HA .
	manualset3
227228	3	421197	7	NULL	NULL	0	NULL	v1 regions	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Despite these differences , second-derivative analysis of the v1 , v3 regions revealed no significant changes in the positions of the underlying bands used to characterize the environments of the phosphate ion in poorly crystalline HA .
	manualset3
227229	4	421197	7	NULL	NULL	0	NULL	v3 regions	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Despite these differences , second-derivative analysis of the v1 , v3 regions revealed no significant changes in the positions of the underlying bands used to characterize the environments of the phosphate ion in poorly crystalline HA .
	manualset3
227230	5	421197	7	NULL	NULL	0	NULL	no significant changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Despite these differences , second-derivative analysis of the v1 , v3 regions revealed no significant changes in the positions of the underlying bands used to characterize the environments of the phosphate ion in poorly crystalline HA .
	manualset3
227231	6	421197	7	NULL	NULL	0	NULL	 positions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Despite these differences , second-derivative analysis of the v1 , v3 regions revealed no significant changes in the positions of the underlying bands used to characterize the environments of the phosphate ion in poorly crystalline HA .
	manualset3
227232	7	421197	7	NULL	NULL	0	NULL	underlying bands	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Despite these differences , second-derivative analysis of the v1 , v3 regions revealed no significant changes in the positions of the underlying bands used to characterize the environments of the phosphate ion in poorly crystalline HA .
	manualset3
227233	8	421197	7	NULL	NULL	0	NULL	environments 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Despite these differences , second-derivative analysis of the v1 , v3 regions revealed no significant changes in the positions of the underlying bands used to characterize the environments of the phosphate ion in poorly crystalline HA .
	manualset3
227234	9	421197	7	NULL	NULL	0	NULL	 phosphate ion	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Despite these differences , second-derivative analysis of the v1 , v3 regions revealed no significant changes in the positions of the underlying bands used to characterize the environments of the phosphate ion in poorly crystalline HA .
	manualset3
227235	10	421197	7	NULL	NULL	0	NULL	crystalline HA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Despite these differences , second-derivative analysis of the v1 , v3 regions revealed no significant changes in the positions of the underlying bands used to characterize the environments of the phosphate ion in poorly crystalline HA .
	manualset3
227236	1	421198	7	NULL	NULL	0	NULL	Specific binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific binding of 125I-insulin-like growth factor I to homogenates prepared from cerebral cortex of Alzheimer 's , alcoholic , alcoholic Alzheimer 's , and age-matched control patients was similar , although Alzheimer 's patients tended to have slightly higher binding values .
	manualset3
227237	2	421198	7	NULL	NULL	0	NULL	125I-insulin-like growth factor I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific binding of 125I-insulin-like growth factor I to homogenates prepared from cerebral cortex of Alzheimer 's , alcoholic , alcoholic Alzheimer 's , and age-matched control patients was similar , although Alzheimer 's patients tended to have slightly higher binding values .
	manualset3
227238	3	421198	7	NULL	NULL	0	NULL	homogenates	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific binding of 125I-insulin-like growth factor I to homogenates prepared from cerebral cortex of Alzheimer 's , alcoholic , alcoholic Alzheimer 's , and age-matched control patients was similar , although Alzheimer 's patients tended to have slightly higher binding values .
	manualset3
227239	4	421198	7	NULL	NULL	0	NULL	 cerebral cortex 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific binding of 125I-insulin-like growth factor I to homogenates prepared from cerebral cortex of Alzheimer 's , alcoholic , alcoholic Alzheimer 's , and age-matched control patients was similar , although Alzheimer 's patients tended to have slightly higher binding values .
	manualset3
227240	5	421198	7	NULL	NULL	NULL	NULL	Alzheimer 's patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Specific binding of 125I-insulin-like growth factor I to homogenates prepared from cerebral cortex of Alzheimer 's , alcoholic , alcoholic Alzheimer 's , and age-matched control patients was similar , although Alzheimer 's patients tended to have slightly higher binding values .
	manualset3
227241	6	421198	7	NULL	NULL	0	NULL	alcoholic Alzheimer 's patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific binding of 125I-insulin-like growth factor I to homogenates prepared from cerebral cortex of Alzheimer 's , alcoholic , alcoholic Alzheimer 's , and age-matched control patients was similar , although Alzheimer 's patients tended to have slightly higher binding values .
	manualset3
227242	7	421198	7	NULL	NULL	0	NULL	age-matched control patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific binding of 125I-insulin-like growth factor I to homogenates prepared from cerebral cortex of Alzheimer 's , alcoholic , alcoholic Alzheimer 's , and age-matched control patients was similar , although Alzheimer 's patients tended to have slightly higher binding values .
	manualset3
227243	8	421198	7	NULL	NULL	0	NULL	alcoholic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific binding of 125I-insulin-like growth factor I to homogenates prepared from cerebral cortex of Alzheimer 's , alcoholic , alcoholic Alzheimer 's , and age-matched control patients was similar , although Alzheimer 's patients tended to have slightly higher binding values .
	manualset3
227244	9	421198	7	NULL	NULL	0	NULL	Alzheimer 's patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific binding of 125I-insulin-like growth factor I to homogenates prepared from cerebral cortex of Alzheimer 's , alcoholic , alcoholic Alzheimer 's , and age-matched control patients was similar , although Alzheimer 's patients tended to have slightly higher binding values .
	manualset3
227245	10	421198	7	NULL	NULL	0	NULL	binding values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific binding of 125I-insulin-like growth factor I to homogenates prepared from cerebral cortex of Alzheimer 's , alcoholic , alcoholic Alzheimer 's , and age-matched control patients was similar , although Alzheimer 's patients tended to have slightly higher binding values .
	manualset3
227246	1	421199	7	NULL	NULL	0	NULL	neurons 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , these neurons were termed ` place cells ' and a theory was developed that suggested that the hippocampus acts as a ` cognitive map ' that is required for spatial orientation .
	manualset3
227247	2	421199	7	NULL	NULL	0	NULL	 place cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , these neurons were termed ` place cells ' and a theory was developed that suggested that the hippocampus acts as a ` cognitive map ' that is required for spatial orientation .
	manualset3
227248	3	421199	7	NULL	NULL	0	NULL	theory	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , these neurons were termed ` place cells ' and a theory was developed that suggested that the hippocampus acts as a ` cognitive map ' that is required for spatial orientation .
	manualset3
227249	4	421199	7	NULL	NULL	0	NULL	hippocampus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , these neurons were termed ` place cells ' and a theory was developed that suggested that the hippocampus acts as a ` cognitive map ' that is required for spatial orientation .
	manualset3
227250	5	421199	7	NULL	NULL	0	NULL	 ` cognitive map ' 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , these neurons were termed ` place cells ' and a theory was developed that suggested that the hippocampus acts as a ` cognitive map ' that is required for spatial orientation .
	manualset3
227251	6	421199	7	NULL	NULL	0	NULL	spatial orientation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , these neurons were termed ` place cells ' and a theory was developed that suggested that the hippocampus acts as a ` cognitive map ' that is required for spatial orientation .
	manualset3
227252	1	421200	7	NULL	NULL	0	NULL	fascicles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphologically , the fascicles had the characteristics of striated muscle ; and , while most were of normal dimensions , several were made up of small fibers 4-10 micron in diameter .
	manualset3
227253	2	421200	7	NULL	NULL	0	NULL	striated muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphologically , the fascicles had the characteristics of striated muscle ; and , while most were of normal dimensions , several were made up of small fibers 4-10 micron in diameter .
	manualset3
227254	3	421200	7	NULL	NULL	0	NULL	normal dimensions	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphologically , the fascicles had the characteristics of striated muscle ; and , while most were of normal dimensions , several were made up of small fibers 4-10 micron in diameter .
	manualset3
227255	4	421200	7	NULL	NULL	0	NULL	small fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphologically , the fascicles had the characteristics of striated muscle ; and , while most were of normal dimensions , several were made up of small fibers 4-10 micron in diameter .
	manualset3
227256	5	421200	7	NULL	NULL	0	NULL	4-10 micron	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphologically , the fascicles had the characteristics of striated muscle ; and , while most were of normal dimensions , several were made up of small fibers 4-10 micron in diameter .
	manualset3
227257	6	421200	7	NULL	NULL	0	NULL	diameter	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Morphologically , the fascicles had the characteristics of striated muscle ; and , while most were of normal dimensions , several were made up of small fibers 4-10 micron in diameter .
	manualset3
227258	1	421201	7	NULL	NULL	0	NULL	 thallium-201 myocardial perfusion scintigraphy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , thallium-201 myocardial perfusion scintigraphy is able to reveal non-invasively right ventricular hypertrophy in patients with chronic pulmonary disease , and it might be a useful means of clinically diagnosing chronic cor pulmonale .
	manualset3
227259	2	421201	7	NULL	NULL	0	NULL	 non-invasively right ventricular hypertrophy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , thallium-201 myocardial perfusion scintigraphy is able to reveal non-invasively right ventricular hypertrophy in patients with chronic pulmonary disease , and it might be a useful means of clinically diagnosing chronic cor pulmonale .
	manualset3
227260	3	421201	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , thallium-201 myocardial perfusion scintigraphy is able to reveal non-invasively right ventricular hypertrophy in patients with chronic pulmonary disease , and it might be a useful means of clinically diagnosing chronic cor pulmonale .
	manualset3
227261	4	421201	7	NULL	NULL	0	NULL	chronic pulmonary disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , thallium-201 myocardial perfusion scintigraphy is able to reveal non-invasively right ventricular hypertrophy in patients with chronic pulmonary disease , and it might be a useful means of clinically diagnosing chronic cor pulmonale .
	manualset3
227262	5	421201	7	NULL	NULL	0	NULL	 useful	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , thallium-201 myocardial perfusion scintigraphy is able to reveal non-invasively right ventricular hypertrophy in patients with chronic pulmonary disease , and it might be a useful means of clinically diagnosing chronic cor pulmonale .
	manualset3
227263	6	421201	7	NULL	NULL	0	NULL	chronic cor pulmonale	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , thallium-201 myocardial perfusion scintigraphy is able to reveal non-invasively right ventricular hypertrophy in patients with chronic pulmonary disease , and it might be a useful means of clinically diagnosing chronic cor pulmonale .
	manualset3
227264	1	421202	7	NULL	NULL	0	NULL	hepatic aryl hydrocarbon hydroxylase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The hepatic aryl hydrocarbon hydroxylase and p-nitroanisole O-demethylase activities decreased in fatty acid-treated rats .
	manualset3
227265	2	421202	7	NULL	NULL	0	NULL	p-nitroanisole O-demethylase activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The hepatic aryl hydrocarbon hydroxylase and p-nitroanisole O-demethylase activities decreased in fatty acid-treated rats .
	manualset3
227266	3	421202	7	NULL	NULL	0	NULL	fatty acid-treated rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The hepatic aryl hydrocarbon hydroxylase and p-nitroanisole O-demethylase activities decreased in fatty acid-treated rats .
	manualset3
227267	1	421203	7	NULL	NULL	0	NULL	Implications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Implications for immunoconjugate therapy , limitations of the approach , and future directions of the research program are discussed .
	manualset3
227268	2	421203	7	NULL	NULL	0	NULL	immunoconjugate therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Implications for immunoconjugate therapy , limitations of the approach , and future directions of the research program are discussed .
	manualset3
227269	3	421203	7	NULL	NULL	0	NULL	 limitations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Implications for immunoconjugate therapy , limitations of the approach , and future directions of the research program are discussed .
	manualset3
227270	4	421203	7	NULL	NULL	0	NULL	 approach	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Implications for immunoconjugate therapy , limitations of the approach , and future directions of the research program are discussed .
	manualset3
227271	5	421203	7	NULL	NULL	0	NULL	future directions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Implications for immunoconjugate therapy , limitations of the approach , and future directions of the research program are discussed .
	manualset3
227272	6	421203	7	NULL	NULL	0	NULL	research program	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Implications for immunoconjugate therapy , limitations of the approach , and future directions of the research program are discussed .
	manualset3
227273	1	421204	7	NULL	NULL	0	NULL	Continuous on-line hydrogen ion monitoring	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuous on-line hydrogen ion monitoring to study flow dynamics of perifusion systems and cellular metabolism .
	manualset3
227274	2	421204	7	NULL	NULL	0	NULL	flow dynamics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuous on-line hydrogen ion monitoring to study flow dynamics of perifusion systems and cellular metabolism .
	manualset3
227275	3	421204	7	NULL	NULL	NULL	NULL	perifusion systems	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Continuous on-line hydrogen ion monitoring to study flow dynamics of perifusion systems and cellular metabolism .
	manualset3
227276	4	421204	7	NULL	NULL	0	NULL	cellular metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuous on-line hydrogen ion monitoring to study flow dynamics of perifusion systems and cellular metabolism .
	manualset3
227277	1	421205	7	NULL	NULL	0	NULL	case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In our case , spinal cord infarction was caused by a massive amount of cholesterol crystals from the aorta related to IABP .
	manualset3
227278	2	421205	7	NULL	NULL	0	NULL	 spinal cord infarction	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In our case , spinal cord infarction was caused by a massive amount of cholesterol crystals from the aorta related to IABP .
	manualset3
227279	3	421205	7	NULL	NULL	0	NULL	massive amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In our case , spinal cord infarction was caused by a massive amount of cholesterol crystals from the aorta related to IABP .
	manualset3
227280	4	421205	7	NULL	NULL	0	NULL	cholesterol crystals 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In our case , spinal cord infarction was caused by a massive amount of cholesterol crystals from the aorta related to IABP .
	manualset3
227281	5	421205	7	NULL	NULL	0	NULL	aorta	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In our case , spinal cord infarction was caused by a massive amount of cholesterol crystals from the aorta related to IABP .
	manualset3
227282	6	421205	7	NULL	NULL	0	NULL	IABP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In our case , spinal cord infarction was caused by a massive amount of cholesterol crystals from the aorta related to IABP .
	manualset3
227283	1	421206	7	NULL	NULL	0	NULL	college	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	However , during college , women tend to reduce their levels of physical activity .
	manualset3
227284	2	421206	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	However , during college , women tend to reduce their levels of physical activity .
	manualset3
227285	3	421206	7	NULL	NULL	0	NULL	levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , during college , women tend to reduce their levels of physical activity .
	manualset3
227286	4	421206	7	NULL	NULL	0	NULL	physical activity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , during college , women tend to reduce their levels of physical activity .
	manualset3
227287	1	421207	7	NULL	NULL	0	NULL	blood pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The blood pressure recovered when the transfusion was stopped and did not decrease any further after restarting the transfusion , were found out not to increase or decrease consistently , and only modest changes in plasma potassium were observed .
	manualset3
227288	2	421207	7	NULL	NULL	0	NULL	transfusion 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The blood pressure recovered when the transfusion was stopped and did not decrease any further after restarting the transfusion , were found out not to increase or decrease consistently , and only modest changes in plasma potassium were observed .
	manualset3
227289	3	421207	7	NULL	NULL	0	NULL	transfusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The blood pressure recovered when the transfusion was stopped and did not decrease any further after restarting the transfusion , were found out not to increase or decrease consistently , and only modest changes in plasma potassium were observed .
	manualset3
227290	4	421207	7	NULL	NULL	0	NULL	 modest changes 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The blood pressure recovered when the transfusion was stopped and did not decrease any further after restarting the transfusion , were found out not to increase or decrease consistently , and only modest changes in plasma potassium were observed .
	manualset3
227291	5	421207	7	NULL	NULL	0	NULL	plasma potassium 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The blood pressure recovered when the transfusion was stopped and did not decrease any further after restarting the transfusion , were found out not to increase or decrease consistently , and only modest changes in plasma potassium were observed .
	manualset3
227292	1	421208	7	NULL	NULL	0	NULL	second study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A second study is underway with greater patient numbers recruited from peripheral hospitals and with an increased period of octreotide medication ( 21 days ) .
	manualset3
227293	2	421208	7	NULL	NULL	0	NULL	patient numbers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A second study is underway with greater patient numbers recruited from peripheral hospitals and with an increased period of octreotide medication ( 21 days ) .
	manualset3
227294	3	421208	7	NULL	NULL	0	NULL	peripheral hospitals	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A second study is underway with greater patient numbers recruited from peripheral hospitals and with an increased period of octreotide medication ( 21 days ) .
	manualset3
227295	4	421208	7	NULL	NULL	0	NULL	 increased period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A second study is underway with greater patient numbers recruited from peripheral hospitals and with an increased period of octreotide medication ( 21 days ) .
	manualset3
227296	5	421208	7	NULL	NULL	0	NULL	octreotide medication	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A second study is underway with greater patient numbers recruited from peripheral hospitals and with an increased period of octreotide medication ( 21 days ) .
	manualset3
227297	6	421208	7	NULL	NULL	0	NULL	21 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A second study is underway with greater patient numbers recruited from peripheral hospitals and with an increased period of octreotide medication ( 21 days ) .
	manualset3
227298	1	421209	7	NULL	NULL	0	NULL	comparative analysis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative analysis of fin phenotypes obtained after retinoic acid treatment or altering the hedgehog signaling levels during regeneration allowed us to assign a limb tetrapod equivalent segment to Polypterus fin skeletal structures , thus providing clues to the origin of the autopod .
	manualset3
227299	2	421209	7	NULL	NULL	0	NULL	fin phenotypes	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative analysis of fin phenotypes obtained after retinoic acid treatment or altering the hedgehog signaling levels during regeneration allowed us to assign a limb tetrapod equivalent segment to Polypterus fin skeletal structures , thus providing clues to the origin of the autopod .
	manualset3
227300	3	421209	7	NULL	NULL	0	NULL	retinoic acid treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative analysis of fin phenotypes obtained after retinoic acid treatment or altering the hedgehog signaling levels during regeneration allowed us to assign a limb tetrapod equivalent segment to Polypterus fin skeletal structures , thus providing clues to the origin of the autopod .
	manualset3
227301	4	421209	7	NULL	NULL	0	NULL	 hedgehog signaling levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative analysis of fin phenotypes obtained after retinoic acid treatment or altering the hedgehog signaling levels during regeneration allowed us to assign a limb tetrapod equivalent segment to Polypterus fin skeletal structures , thus providing clues to the origin of the autopod .
	manualset3
227302	5	421209	7	NULL	NULL	0	NULL	regeneration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative analysis of fin phenotypes obtained after retinoic acid treatment or altering the hedgehog signaling levels during regeneration allowed us to assign a limb tetrapod equivalent segment to Polypterus fin skeletal structures , thus providing clues to the origin of the autopod .
	manualset3
227303	6	421209	7	NULL	NULL	0	NULL	limb tetrapod	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative analysis of fin phenotypes obtained after retinoic acid treatment or altering the hedgehog signaling levels during regeneration allowed us to assign a limb tetrapod equivalent segment to Polypterus fin skeletal structures , thus providing clues to the origin of the autopod .
	manualset3
227304	7	421209	7	NULL	NULL	0	NULL	Polypterus fin skeletal structures	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative analysis of fin phenotypes obtained after retinoic acid treatment or altering the hedgehog signaling levels during regeneration allowed us to assign a limb tetrapod equivalent segment to Polypterus fin skeletal structures , thus providing clues to the origin of the autopod .
	manualset3
227305	8	421209	7	NULL	NULL	0	NULL	clues 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative analysis of fin phenotypes obtained after retinoic acid treatment or altering the hedgehog signaling levels during regeneration allowed us to assign a limb tetrapod equivalent segment to Polypterus fin skeletal structures , thus providing clues to the origin of the autopod .
	manualset3
227306	9	421209	7	NULL	NULL	0	NULL	origin	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative analysis of fin phenotypes obtained after retinoic acid treatment or altering the hedgehog signaling levels during regeneration allowed us to assign a limb tetrapod equivalent segment to Polypterus fin skeletal structures , thus providing clues to the origin of the autopod .
	manualset3
227307	10	421209	7	NULL	NULL	0	NULL	autopod	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A comparative analysis of fin phenotypes obtained after retinoic acid treatment or altering the hedgehog signaling levels during regeneration allowed us to assign a limb tetrapod equivalent segment to Polypterus fin skeletal structures , thus providing clues to the origin of the autopod .
	manualset3
227308	1	421210	7	NULL	NULL	0	NULL	Determination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of operability of bronchial cancer by angiopneumography ; present state of the problem ) .
	manualset3
227309	2	421210	7	NULL	NULL	0	NULL	operability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of operability of bronchial cancer by angiopneumography ; present state of the problem ) .
	manualset3
227310	3	421210	7	NULL	NULL	0	NULL	bronchial cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of operability of bronchial cancer by angiopneumography ; present state of the problem ) .
	manualset3
227311	4	421210	7	NULL	NULL	0	NULL	angiopneumography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of operability of bronchial cancer by angiopneumography ; present state of the problem ) .
	manualset3
227312	5	421210	7	NULL	NULL	0	NULL	 present state	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of operability of bronchial cancer by angiopneumography ; present state of the problem ) .
	manualset3
227313	6	421210	7	NULL	NULL	0	NULL	 problem	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of operability of bronchial cancer by angiopneumography ; present state of the problem ) .
	manualset3
227314	1	421211	7	NULL	NULL	0	NULL	Results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest an acceptable factor structure and reliability .
	manualset3
227315	2	421211	7	NULL	NULL	0	NULL	acceptable factor structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest an acceptable factor structure and reliability .
	manualset3
227316	3	421211	7	NULL	NULL	0	NULL	reliability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Results suggest an acceptable factor structure and reliability .
	manualset3
227317	1	421212	7	NULL	NULL	0	NULL	Fetal placental tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Fetal placental tissue from 11 days pregnant mice was dissociated in collagenase and DNase solution and then separated on a 40 per cent Percoll gradient .
	manualset3
227318	2	421212	7	NULL	NULL	0	NULL	11 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Fetal placental tissue from 11 days pregnant mice was dissociated in collagenase and DNase solution and then separated on a 40 per cent Percoll gradient .
	manualset3
227319	3	421212	7	NULL	NULL	0	NULL	pregnant mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Fetal placental tissue from 11 days pregnant mice was dissociated in collagenase and DNase solution and then separated on a 40 per cent Percoll gradient .
	manualset3
227320	4	421212	7	NULL	NULL	0	NULL	 collagenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Fetal placental tissue from 11 days pregnant mice was dissociated in collagenase and DNase solution and then separated on a 40 per cent Percoll gradient .
	manualset3
227321	5	421212	7	NULL	NULL	0	NULL	DNase solution	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Fetal placental tissue from 11 days pregnant mice was dissociated in collagenase and DNase solution and then separated on a 40 per cent Percoll gradient .
	manualset3
227322	6	421212	7	NULL	NULL	0	NULL	40 per cent	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Fetal placental tissue from 11 days pregnant mice was dissociated in collagenase and DNase solution and then separated on a 40 per cent Percoll gradient .
	manualset3
227323	7	421212	7	NULL	NULL	0	NULL	Percoll gradient	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Fetal placental tissue from 11 days pregnant mice was dissociated in collagenase and DNase solution and then separated on a 40 per cent Percoll gradient .
	manualset3
227324	1	421213	7	NULL	NULL	0	NULL	conclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , alkyl substitution in the 2-position of idazoxan can enhance either alpha 2-adrenoceptor antagonist potency or selectivity or both and furthermore , the weak partial alpha 1-adrenoceptor agonist properties of idazoxan can be removed .
	manualset3
227325	2	421213	7	NULL	NULL	0	NULL	alkyl substitution 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , alkyl substitution in the 2-position of idazoxan can enhance either alpha 2-adrenoceptor antagonist potency or selectivity or both and furthermore , the weak partial alpha 1-adrenoceptor agonist properties of idazoxan can be removed .
	manualset3
227326	3	421213	7	NULL	NULL	0	NULL	 2-position	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , alkyl substitution in the 2-position of idazoxan can enhance either alpha 2-adrenoceptor antagonist potency or selectivity or both and furthermore , the weak partial alpha 1-adrenoceptor agonist properties of idazoxan can be removed .
	manualset3
227327	4	421213	7	NULL	NULL	0	NULL	idazoxan	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , alkyl substitution in the 2-position of idazoxan can enhance either alpha 2-adrenoceptor antagonist potency or selectivity or both and furthermore , the weak partial alpha 1-adrenoceptor agonist properties of idazoxan can be removed .
	manualset3
227328	5	421213	7	NULL	NULL	0	NULL	alpha 2-adrenoceptor antagonist potency	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , alkyl substitution in the 2-position of idazoxan can enhance either alpha 2-adrenoceptor antagonist potency or selectivity or both and furthermore , the weak partial alpha 1-adrenoceptor agonist properties of idazoxan can be removed .
	manualset3
227329	6	421213	7	NULL	NULL	0	NULL	weak partial alpha 1-adrenoceptor agonist properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , alkyl substitution in the 2-position of idazoxan can enhance either alpha 2-adrenoceptor antagonist potency or selectivity or both and furthermore , the weak partial alpha 1-adrenoceptor agonist properties of idazoxan can be removed .
	manualset3
227330	7	421213	7	NULL	NULL	0	NULL	idazoxan	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , alkyl substitution in the 2-position of idazoxan can enhance either alpha 2-adrenoceptor antagonist potency or selectivity or both and furthermore , the weak partial alpha 1-adrenoceptor agonist properties of idazoxan can be removed .
	manualset3
227331	1	421214	7	NULL	NULL	0	NULL	nitrogen monoxide ( NO ) concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased nitrogen monoxide ( NO ) concentrations change leukocyte function under a multitude of experimental conditions .
	manualset3
227332	2	421214	7	NULL	NULL	0	NULL	 leukocyte function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased nitrogen monoxide ( NO ) concentrations change leukocyte function under a multitude of experimental conditions .
	manualset3
227333	3	421214	7	NULL	NULL	0	NULL	 multitude	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased nitrogen monoxide ( NO ) concentrations change leukocyte function under a multitude of experimental conditions .
	manualset3
227334	4	421214	7	NULL	NULL	0	NULL	experimental conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased nitrogen monoxide ( NO ) concentrations change leukocyte function under a multitude of experimental conditions .
	manualset3
227505	1	421215	7	NULL	NULL	0	NULL	changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneously with the changes in expression of the extracellular matrix proteins , the expression pattern of basic fibroblast growth factor ( FGF-2 ) was markedly altered after spinal cord injury .
	manualset3
227507	2	421215	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneously with the changes in expression of the extracellular matrix proteins , the expression pattern of basic fibroblast growth factor ( FGF-2 ) was markedly altered after spinal cord injury .
	manualset3
227508	3	421215	7	NULL	NULL	0	NULL	extracellular matrix proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneously with the changes in expression of the extracellular matrix proteins , the expression pattern of basic fibroblast growth factor ( FGF-2 ) was markedly altered after spinal cord injury .
	manualset3
227510	4	421215	7	NULL	NULL	0	NULL	expression pattern	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneously with the changes in expression of the extracellular matrix proteins , the expression pattern of basic fibroblast growth factor ( FGF-2 ) was markedly altered after spinal cord injury .
	manualset3
227512	5	421215	7	NULL	NULL	0	NULL	basic fibroblast growth factor ( FGF-2 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneously with the changes in expression of the extracellular matrix proteins , the expression pattern of basic fibroblast growth factor ( FGF-2 ) was markedly altered after spinal cord injury .
	manualset3
227513	6	421215	7	NULL	NULL	0	NULL	spinal cord injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Simultaneously with the changes in expression of the extracellular matrix proteins , the expression pattern of basic fibroblast growth factor ( FGF-2 ) was markedly altered after spinal cord injury .
	manualset3
227515	1	421216	7	NULL	NULL	0	NULL	Bone substitutes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Bone substitutes do not provide the cellular elements necessary for osteogenesis , and they can not be considered osteoinductive , but instead are osteoconductive , providing a scaffold for new bone deposition .
	manualset3
227518	2	421216	7	NULL	NULL	0	NULL	cellular elements	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Bone substitutes do not provide the cellular elements necessary for osteogenesis , and they can not be considered osteoinductive , but instead are osteoconductive , providing a scaffold for new bone deposition .
	manualset3
227521	3	421216	7	NULL	NULL	0	NULL	osteogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Bone substitutes do not provide the cellular elements necessary for osteogenesis , and they can not be considered osteoinductive , but instead are osteoconductive , providing a scaffold for new bone deposition .
	manualset3
227522	4	421216	7	NULL	NULL	0	NULL	scaffold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Bone substitutes do not provide the cellular elements necessary for osteogenesis , and they can not be considered osteoinductive , but instead are osteoconductive , providing a scaffold for new bone deposition .
	manualset3
227523	5	421216	7	NULL	NULL	0	NULL	new bone deposition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Bone substitutes do not provide the cellular elements necessary for osteogenesis , and they can not be considered osteoinductive , but instead are osteoconductive , providing a scaffold for new bone deposition .
	manualset3
227524	1	421217	7	NULL	NULL	0	NULL	 779 medical records	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	We analyzed 779 medical records of patients bitten by B. jararaca and treated at the Hospital Vital Brazil , Butantan Institute , So Paulo , Brazil , between 1982 and 1990 : 111 cases with necrosis were compared with the remaining cases .
	manualset3
227525	2	421217	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We analyzed 779 medical records of patients bitten by B. jararaca and treated at the Hospital Vital Brazil , Butantan Institute , So Paulo , Brazil , between 1982 and 1990 : 111 cases with necrosis were compared with the remaining cases .
	manualset3
227527	3	421217	7	NULL	NULL	0	NULL	B. jararaca	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We analyzed 779 medical records of patients bitten by B. jararaca and treated at the Hospital Vital Brazil , Butantan Institute , So Paulo , Brazil , between 1982 and 1990 : 111 cases with necrosis were compared with the remaining cases .
	manualset3
227528	4	421217	7	NULL	NULL	0	NULL	Hospital Vital Brazil 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	We analyzed 779 medical records of patients bitten by B. jararaca and treated at the Hospital Vital Brazil , Butantan Institute , So Paulo , Brazil , between 1982 and 1990 : 111 cases with necrosis were compared with the remaining cases .
	manualset3
227529	5	421217	7	NULL	NULL	0	NULL	Butantan Institute	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	We analyzed 779 medical records of patients bitten by B. jararaca and treated at the Hospital Vital Brazil , Butantan Institute , So Paulo , Brazil , between 1982 and 1990 : 111 cases with necrosis were compared with the remaining cases .
	manualset3
227531	6	421217	7	NULL	NULL	0	NULL	So Paulo ,	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	We analyzed 779 medical records of patients bitten by B. jararaca and treated at the Hospital Vital Brazil , Butantan Institute , So Paulo , Brazil , between 1982 and 1990 : 111 cases with necrosis were compared with the remaining cases .
	manualset3
227533	7	421217	7	NULL	NULL	0	NULL	Brazil	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	We analyzed 779 medical records of patients bitten by B. jararaca and treated at the Hospital Vital Brazil , Butantan Institute , So Paulo , Brazil , between 1982 and 1990 : 111 cases with necrosis were compared with the remaining cases .
	manualset3
227534	8	421217	7	NULL	NULL	0	NULL	1982	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	We analyzed 779 medical records of patients bitten by B. jararaca and treated at the Hospital Vital Brazil , Butantan Institute , So Paulo , Brazil , between 1982 and 1990 : 111 cases with necrosis were compared with the remaining cases .
	manualset3
227536	9	421217	7	NULL	NULL	0	NULL	 1990	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	We analyzed 779 medical records of patients bitten by B. jararaca and treated at the Hospital Vital Brazil , Butantan Institute , So Paulo , Brazil , between 1982 and 1990 : 111 cases with necrosis were compared with the remaining cases .
	manualset3
227539	10	421217	7	NULL	NULL	0	NULL	111 cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We analyzed 779 medical records of patients bitten by B. jararaca and treated at the Hospital Vital Brazil , Butantan Institute , So Paulo , Brazil , between 1982 and 1990 : 111 cases with necrosis were compared with the remaining cases .
	manualset3
227541	11	421217	7	NULL	NULL	0	NULL	necrosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We analyzed 779 medical records of patients bitten by B. jararaca and treated at the Hospital Vital Brazil , Butantan Institute , So Paulo , Brazil , between 1982 and 1990 : 111 cases with necrosis were compared with the remaining cases .
	manualset3
227542	12	421217	7	NULL	NULL	0	NULL	 cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We analyzed 779 medical records of patients bitten by B. jararaca and treated at the Hospital Vital Brazil , Butantan Institute , So Paulo , Brazil , between 1982 and 1990 : 111 cases with necrosis were compared with the remaining cases .
	manualset3
227543	1	421218	7	NULL	NULL	0	NULL	Amputees 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Amputees and sports : a systematic review .
	manualset3
227545	2	421218	7	NULL	NULL	0	NULL	sports	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Amputees and sports : a systematic review .
	manualset3
227546	3	421218	7	NULL	NULL	0	NULL	systematic review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Amputees and sports : a systematic review .
	manualset3
227549	1	421219	7	NULL	NULL	0	NULL	 Fatal pulmonary fibrosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Fatal pulmonary fibrosis caused by gold therapy ? ) .
	manualset3
227551	2	421219	7	NULL	NULL	0	NULL	 gold therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Fatal pulmonary fibrosis caused by gold therapy ? ) .
	manualset3
227553	1	421220	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship of treadmill test performance to blood pressure and other cardiovascular risk factors in adolescents .
	manualset3
227555	2	421220	7	NULL	NULL	0	NULL	treadmill test performance	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship of treadmill test performance to blood pressure and other cardiovascular risk factors in adolescents .
	manualset3
227557	3	421220	7	NULL	NULL	0	NULL	blood pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship of treadmill test performance to blood pressure and other cardiovascular risk factors in adolescents .
	manualset3
227558	4	421220	7	NULL	NULL	0	NULL	cardiovascular risk factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship of treadmill test performance to blood pressure and other cardiovascular risk factors in adolescents .
	manualset3
227559	5	421220	7	NULL	NULL	0	NULL	adolescents 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The relationship of treadmill test performance to blood pressure and other cardiovascular risk factors in adolescents .
	manualset3
227560	1	421221	7	NULL	NULL	0	NULL	Significance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Significance of estradiol in the development of fibrosis in systemic scleroderma ( bases of sexual predisposition to the disease ) ) .
	manualset3
227562	2	421221	7	NULL	NULL	0	NULL	estradiol 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Significance of estradiol in the development of fibrosis in systemic scleroderma ( bases of sexual predisposition to the disease ) ) .
	manualset3
227564	3	421221	7	NULL	NULL	0	NULL	 development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Significance of estradiol in the development of fibrosis in systemic scleroderma ( bases of sexual predisposition to the disease ) ) .
	manualset3
227565	4	421221	7	NULL	NULL	0	NULL	 fibrosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Significance of estradiol in the development of fibrosis in systemic scleroderma ( bases of sexual predisposition to the disease ) ) .
	manualset3
227567	5	421221	7	NULL	NULL	0	NULL	 systemic scleroderma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Significance of estradiol in the development of fibrosis in systemic scleroderma ( bases of sexual predisposition to the disease ) ) .
	manualset3
227568	6	421221	7	NULL	NULL	0	NULL	bases	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Significance of estradiol in the development of fibrosis in systemic scleroderma ( bases of sexual predisposition to the disease ) ) .
	manualset3
227569	7	421221	7	NULL	NULL	0	NULL	sexual predisposition 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Significance of estradiol in the development of fibrosis in systemic scleroderma ( bases of sexual predisposition to the disease ) ) .
	manualset3
227570	8	421221	7	NULL	NULL	0	NULL	 disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Significance of estradiol in the development of fibrosis in systemic scleroderma ( bases of sexual predisposition to the disease ) ) .
	manualset3
227572	1	421222	7	NULL	NULL	0	NULL	Adenosine 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenosine remains the drug of choice in the treatment of paroxysmal supraventricular tachycardia .
	manualset3
227574	2	421222	7	NULL	NULL	0	NULL	drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenosine remains the drug of choice in the treatment of paroxysmal supraventricular tachycardia .
	manualset3
227575	3	421222	7	NULL	NULL	0	NULL	 treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenosine remains the drug of choice in the treatment of paroxysmal supraventricular tachycardia .
	manualset3
227576	4	421222	7	NULL	NULL	0	NULL	paroxysmal supraventricular tachycardia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Adenosine remains the drug of choice in the treatment of paroxysmal supraventricular tachycardia .
	manualset3
227579	1	421223	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of different excitation wavelength allows us to emphasize the selectivity of the process and to identify the active role of the 2 ( 1 ) Ag state in this pressure - and laser-induced chemical reaction .
	manualset3
227580	2	421223	7	NULL	NULL	0	NULL	different excitation wavelength	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of different excitation wavelength allows us to emphasize the selectivity of the process and to identify the active role of the 2 ( 1 ) Ag state in this pressure - and laser-induced chemical reaction .
	manualset3
227587	3	421223	7	NULL	NULL	0	NULL	selectivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of different excitation wavelength allows us to emphasize the selectivity of the process and to identify the active role of the 2 ( 1 ) Ag state in this pressure - and laser-induced chemical reaction .
	manualset3
227588	4	421223	7	NULL	NULL	0	NULL	process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of different excitation wavelength allows us to emphasize the selectivity of the process and to identify the active role of the 2 ( 1 ) Ag state in this pressure - and laser-induced chemical reaction .
	manualset3
227589	5	421223	7	NULL	NULL	0	NULL	active role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of different excitation wavelength allows us to emphasize the selectivity of the process and to identify the active role of the 2 ( 1 ) Ag state in this pressure - and laser-induced chemical reaction .
	manualset3
227591	6	421223	7	NULL	NULL	0	NULL	Ag state	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of different excitation wavelength allows us to emphasize the selectivity of the process and to identify the active role of the 2 ( 1 ) Ag state in this pressure - and laser-induced chemical reaction .
	manualset3
227593	7	421223	7	NULL	NULL	0	NULL	pressure 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of different excitation wavelength allows us to emphasize the selectivity of the process and to identify the active role of the 2 ( 1 ) Ag state in this pressure - and laser-induced chemical reaction .
	manualset3
227595	8	421223	7	NULL	NULL	0	NULL	laser-induced chemical reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The use of different excitation wavelength allows us to emphasize the selectivity of the process and to identify the active role of the 2 ( 1 ) Ag state in this pressure - and laser-induced chemical reaction .
	manualset3
227597	1	421224	7	NULL	NULL	0	NULL	present data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data provide further evidence to support the notion that the serotonergic system is involved in the manifestation of the persistent abnormalities induced by IDPN .
	manualset3
227607	2	421224	7	NULL	NULL	0	NULL	 evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data provide further evidence to support the notion that the serotonergic system is involved in the manifestation of the persistent abnormalities induced by IDPN .
	manualset3
227609	3	421224	7	NULL	NULL	0	NULL	notion	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data provide further evidence to support the notion that the serotonergic system is involved in the manifestation of the persistent abnormalities induced by IDPN .
	manualset3
227610	4	421224	7	NULL	NULL	0	NULL	serotonergic system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data provide further evidence to support the notion that the serotonergic system is involved in the manifestation of the persistent abnormalities induced by IDPN .
	manualset3
227611	5	421224	7	NULL	NULL	0	NULL	manifestation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data provide further evidence to support the notion that the serotonergic system is involved in the manifestation of the persistent abnormalities induced by IDPN .
	manualset3
227612	6	421224	7	NULL	NULL	0	NULL	persistent abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data provide further evidence to support the notion that the serotonergic system is involved in the manifestation of the persistent abnormalities induced by IDPN .
	manualset3
227616	7	421224	7	NULL	NULL	0	NULL	IDPN	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data provide further evidence to support the notion that the serotonergic system is involved in the manifestation of the persistent abnormalities induced by IDPN .
	manualset3
227619	1	421225	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients died of disease within 33 months of diagnosis .
	manualset3
227621	2	421225	7	NULL	NULL	0	NULL	 disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients died of disease within 33 months of diagnosis .
	manualset3
227622	3	421225	7	NULL	NULL	0	NULL	 33 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients died of disease within 33 months of diagnosis .
	manualset3
227623	4	421225	7	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients died of disease within 33 months of diagnosis .
	manualset3
227625	1	421226	7	NULL	NULL	0	NULL	Preliminary evidence 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary evidence indicates that mirror neurons may be involved in theory of mind ; however , these data by their very nature are reliant on the presence , and precise characterization , of the human mirror system .
	manualset3
227631	2	421226	7	NULL	NULL	NULL	NULL	mirror neurons	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Preliminary evidence indicates that mirror neurons may be involved in theory of mind ; however , these data by their very nature are reliant on the presence , and precise characterization , of the human mirror system .
	manualset3
227632	3	421226	7	NULL	NULL	NULL	NULL	 theory of mind 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Preliminary evidence indicates that mirror neurons may be involved in theory of mind ; however , these data by their very nature are reliant on the presence , and precise characterization , of the human mirror system .
	manualset3
227633	4	421226	7	NULL	NULL	NULL	NULL	data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Preliminary evidence indicates that mirror neurons may be involved in theory of mind ; however , these data by their very nature are reliant on the presence , and precise characterization , of the human mirror system .
	manualset3
227636	5	421226	7	NULL	NULL	NULL	NULL	 nature	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Preliminary evidence indicates that mirror neurons may be involved in theory of mind ; however , these data by their very nature are reliant on the presence , and precise characterization , of the human mirror system .
	manualset3
227638	6	421226	7	NULL	NULL	0	NULL	 presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary evidence indicates that mirror neurons may be involved in theory of mind ; however , these data by their very nature are reliant on the presence , and precise characterization , of the human mirror system .
	manualset3
227639	7	421226	7	NULL	NULL	0	NULL	precise characterization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Preliminary evidence indicates that mirror neurons may be involved in theory of mind ; however , these data by their very nature are reliant on the presence , and precise characterization , of the human mirror system .
	manualset3
227640	8	421226	7	NULL	NULL	NULL	NULL	 human mirror system	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Preliminary evidence indicates that mirror neurons may be involved in theory of mind ; however , these data by their very nature are reliant on the presence , and precise characterization , of the human mirror system .
	manualset3
227643	1	421227	7	NULL	NULL	0	NULL	Amylase B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Amylase B is suggested to display a higher Km than amylase A , offering a means of adapting to high substrate concentrations .
	manualset3
227645	2	421227	7	NULL	NULL	0	NULL	higher Km	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Amylase B is suggested to display a higher Km than amylase A , offering a means of adapting to high substrate concentrations .
	manualset3
227647	3	421227	7	NULL	NULL	0	NULL	amylase A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Amylase B is suggested to display a higher Km than amylase A , offering a means of adapting to high substrate concentrations .
	manualset3
227648	4	421227	7	NULL	NULL	0	NULL	 means	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Amylase B is suggested to display a higher Km than amylase A , offering a means of adapting to high substrate concentrations .
	manualset3
227650	5	421227	7	NULL	NULL	0	NULL	high substrate concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Amylase B is suggested to display a higher Km than amylase A , offering a means of adapting to high substrate concentrations .
	manualset3
227655	1	421228	7	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with the classical dosage schedule of levamisole ( 150 mg on 3 consecutive days each week ) a single weekly dose of 150 mg levamisole was found to be slightly less effective but much better tolerated .
	manualset3
227656	2	421228	7	NULL	NULL	0	NULL	 classical dosage schedule	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with the classical dosage schedule of levamisole ( 150 mg on 3 consecutive days each week ) a single weekly dose of 150 mg levamisole was found to be slightly less effective but much better tolerated .
	manualset3
227657	3	421228	7	NULL	NULL	0	NULL	levamisole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with the classical dosage schedule of levamisole ( 150 mg on 3 consecutive days each week ) a single weekly dose of 150 mg levamisole was found to be slightly less effective but much better tolerated .
	manualset3
227658	4	421228	7	NULL	NULL	0	NULL	150 mg	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with the classical dosage schedule of levamisole ( 150 mg on 3 consecutive days each week ) a single weekly dose of 150 mg levamisole was found to be slightly less effective but much better tolerated .
	manualset3
227659	5	421228	7	NULL	NULL	0	NULL	 3 consecutive days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with the classical dosage schedule of levamisole ( 150 mg on 3 consecutive days each week ) a single weekly dose of 150 mg levamisole was found to be slightly less effective but much better tolerated .
	manualset3
227660	6	421228	7	NULL	NULL	0	NULL	week 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with the classical dosage schedule of levamisole ( 150 mg on 3 consecutive days each week ) a single weekly dose of 150 mg levamisole was found to be slightly less effective but much better tolerated .
	manualset3
227662	7	421228	7	NULL	NULL	0	NULL	single weekly dose 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with the classical dosage schedule of levamisole ( 150 mg on 3 consecutive days each week ) a single weekly dose of 150 mg levamisole was found to be slightly less effective but much better tolerated .
	manualset3
227663	8	421228	7	NULL	NULL	0	NULL	150 mg	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with the classical dosage schedule of levamisole ( 150 mg on 3 consecutive days each week ) a single weekly dose of 150 mg levamisole was found to be slightly less effective but much better tolerated .
	manualset3
227665	9	421228	7	NULL	NULL	0	NULL	 levamisole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In comparison with the classical dosage schedule of levamisole ( 150 mg on 3 consecutive days each week ) a single weekly dose of 150 mg levamisole was found to be slightly less effective but much better tolerated .
	manualset3
227669	1	421229	7	NULL	NULL	0	NULL	structural changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We examined the structural changes of capillaries in the rat soleus muscle 4 , 7 , 14 , and 35 days after experimental limb tenotomy .
	manualset3
227670	2	421229	7	NULL	NULL	0	NULL	 capillaries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We examined the structural changes of capillaries in the rat soleus muscle 4 , 7 , 14 , and 35 days after experimental limb tenotomy .
	manualset3
227671	3	421229	7	NULL	NULL	0	NULL	rat soleus muscle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We examined the structural changes of capillaries in the rat soleus muscle 4 , 7 , 14 , and 35 days after experimental limb tenotomy .
	manualset3
227672	4	421229	7	NULL	NULL	0	NULL	4 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	We examined the structural changes of capillaries in the rat soleus muscle 4 , 7 , 14 , and 35 days after experimental limb tenotomy .
	manualset3
227674	5	421229	7	NULL	NULL	0	NULL	7 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	We examined the structural changes of capillaries in the rat soleus muscle 4 , 7 , 14 , and 35 days after experimental limb tenotomy .
	manualset3
227676	6	421229	7	NULL	NULL	0	NULL	14 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	We examined the structural changes of capillaries in the rat soleus muscle 4 , 7 , 14 , and 35 days after experimental limb tenotomy .
	manualset3
227677	7	421229	7	NULL	NULL	0	NULL	 35 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	We examined the structural changes of capillaries in the rat soleus muscle 4 , 7 , 14 , and 35 days after experimental limb tenotomy .
	manualset3
227680	8	421229	7	NULL	NULL	0	NULL	experimental limb tenotomy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	We examined the structural changes of capillaries in the rat soleus muscle 4 , 7 , 14 , and 35 days after experimental limb tenotomy .
	manualset3
227682	1	421230	7	NULL	NULL	0	NULL	Anterograde propagation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Anterograde propagation of BoNT/A effects required axonal transport , ruling out a systemic spread of the toxin .
	manualset3
227684	2	421230	7	NULL	NULL	0	NULL	BoNT/A effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Anterograde propagation of BoNT/A effects required axonal transport , ruling out a systemic spread of the toxin .
	manualset3
227686	3	421230	7	NULL	NULL	0	NULL	axonal transport	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Anterograde propagation of BoNT/A effects required axonal transport , ruling out a systemic spread of the toxin .
	manualset3
227692	4	421230	7	NULL	NULL	0	NULL	systemic spread	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Anterograde propagation of BoNT/A effects required axonal transport , ruling out a systemic spread of the toxin .
	manualset3
227693	5	421230	7	NULL	NULL	0	NULL	toxin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Anterograde propagation of BoNT/A effects required axonal transport , ruling out a systemic spread of the toxin .
	manualset3
227837	1	421231	7	NULL	NULL	0	NULL	coprecipitation studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , coprecipitation studies strongly suggest an interaction between NS4A and the N-terminal region of NS3 .
	manualset3
227838	2	421231	7	NULL	NULL	0	NULL	 interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , coprecipitation studies strongly suggest an interaction between NS4A and the N-terminal region of NS3 .
	manualset3
227839	3	421231	7	NULL	NULL	0	NULL	NS4A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , coprecipitation studies strongly suggest an interaction between NS4A and the N-terminal region of NS3 .
	manualset3
227840	4	421231	7	NULL	NULL	0	NULL	N-terminal region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , coprecipitation studies strongly suggest an interaction between NS4A and the N-terminal region of NS3 .
	manualset3
227841	5	421231	7	NULL	NULL	0	NULL	NS3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , coprecipitation studies strongly suggest an interaction between NS4A and the N-terminal region of NS3 .
	manualset3
227842	1	421232	7	NULL	NULL	0	NULL	Focusing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Focusing on the biological aspects of immunity to diseases such as smallpox , Andrew Noymer demonstrates that infectious diseases alone could not account for the Indios ' population collapse .
	manualset3
227843	2	421232	7	NULL	NULL	NULL	NULL	biological aspects	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Focusing on the biological aspects of immunity to diseases such as smallpox , Andrew Noymer demonstrates that infectious diseases alone could not account for the Indios ' population collapse .
	manualset3
227844	3	421232	7	NULL	NULL	0	NULL	 immunity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Focusing on the biological aspects of immunity to diseases such as smallpox , Andrew Noymer demonstrates that infectious diseases alone could not account for the Indios ' population collapse .
	manualset3
227845	4	421232	7	NULL	NULL	0	NULL	diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Focusing on the biological aspects of immunity to diseases such as smallpox , Andrew Noymer demonstrates that infectious diseases alone could not account for the Indios ' population collapse .
	manualset3
227846	5	421232	7	NULL	NULL	0	NULL	 smallpox	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Focusing on the biological aspects of immunity to diseases such as smallpox , Andrew Noymer demonstrates that infectious diseases alone could not account for the Indios ' population collapse .
	manualset3
227847	6	421232	7	NULL	NULL	0	NULL	Andrew Noymer	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Focusing on the biological aspects of immunity to diseases such as smallpox , Andrew Noymer demonstrates that infectious diseases alone could not account for the Indios ' population collapse .
	manualset3
227848	7	421232	7	NULL	NULL	0	NULL	infectious diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Focusing on the biological aspects of immunity to diseases such as smallpox , Andrew Noymer demonstrates that infectious diseases alone could not account for the Indios ' population collapse .
	manualset3
227849	8	421232	7	NULL	NULL	0	NULL	 Indios ' population 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Focusing on the biological aspects of immunity to diseases such as smallpox , Andrew Noymer demonstrates that infectious diseases alone could not account for the Indios ' population collapse .
	manualset3
227850	9	421232	7	NULL	NULL	0	NULL	collapse	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Focusing on the biological aspects of immunity to diseases such as smallpox , Andrew Noymer demonstrates that infectious diseases alone could not account for the Indios ' population collapse .
	manualset3
227851	1	421233	7	NULL	NULL	0	NULL	Rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were sacrificed on 1st , 2nd , 4th , 6th , and 8th week after initiation of the experiment .
	manualset3
227852	2	421233	7	NULL	NULL	0	NULL	1st week	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were sacrificed on 1st , 2nd , 4th , 6th , and 8th week after initiation of the experiment .
	manualset3
227853	3	421233	7	NULL	NULL	0	NULL	2nd week	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were sacrificed on 1st , 2nd , 4th , 6th , and 8th week after initiation of the experiment .
	manualset3
227854	4	421233	7	NULL	NULL	0	NULL	4th week	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were sacrificed on 1st , 2nd , 4th , 6th , and 8th week after initiation of the experiment .
	manualset3
227855	5	421233	7	NULL	NULL	0	NULL	 6th week	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were sacrificed on 1st , 2nd , 4th , 6th , and 8th week after initiation of the experiment .
	manualset3
227856	6	421233	7	NULL	NULL	0	NULL	8th week	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were sacrificed on 1st , 2nd , 4th , 6th , and 8th week after initiation of the experiment .
	manualset3
227857	7	421233	7	NULL	NULL	0	NULL	initiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were sacrificed on 1st , 2nd , 4th , 6th , and 8th week after initiation of the experiment .
	manualset3
227858	8	421233	7	NULL	NULL	0	NULL	experiment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Rats were sacrificed on 1st , 2nd , 4th , 6th , and 8th week after initiation of the experiment .
	manualset3
227859	1	421234	7	NULL	NULL	0	NULL	Amyloid-beta peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Amyloid-beta peptides are produced by sequential processing of the beta-amyloid precursor protein by the two aspartyl-type proteases beta-secretase and gamma-secretase .
	manualset3
227860	2	421234	7	NULL	NULL	0	NULL	sequential processing	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Amyloid-beta peptides are produced by sequential processing of the beta-amyloid precursor protein by the two aspartyl-type proteases beta-secretase and gamma-secretase .
	manualset3
227861	3	421234	7	NULL	NULL	0	NULL	beta-amyloid precursor protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Amyloid-beta peptides are produced by sequential processing of the beta-amyloid precursor protein by the two aspartyl-type proteases beta-secretase and gamma-secretase .
	manualset3
227862	4	421234	7	NULL	NULL	0	NULL	two aspartyl-type proteases beta-secretase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Amyloid-beta peptides are produced by sequential processing of the beta-amyloid precursor protein by the two aspartyl-type proteases beta-secretase and gamma-secretase .
	manualset3
227863	5	421234	7	NULL	NULL	0	NULL	gamma-secretase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Amyloid-beta peptides are produced by sequential processing of the beta-amyloid precursor protein by the two aspartyl-type proteases beta-secretase and gamma-secretase .
	manualset3
227864	1	421235	7	NULL	NULL	0	NULL	 normal young rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal young rats , 0.05-0 .1 % of ingested aluminium is absorbed in the intestine , of which roughly half goes to the skeleton within 2 h , whereas the remaining half is excreted in the urine , most of it within 48 h. Deposition in organs other than the skeleton appears to be negligible .
	manualset3
227865	2	421235	7	NULL	NULL	0	NULL	0.05-0 .1 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal young rats , 0.05-0 .1 % of ingested aluminium is absorbed in the intestine , of which roughly half goes to the skeleton within 2 h , whereas the remaining half is excreted in the urine , most of it within 48 h. Deposition in organs other than the skeleton appears to be negligible .
	manualset3
227866	3	421235	7	NULL	NULL	0	NULL	ingested aluminium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal young rats , 0.05-0 .1 % of ingested aluminium is absorbed in the intestine , of which roughly half goes to the skeleton within 2 h , whereas the remaining half is excreted in the urine , most of it within 48 h. Deposition in organs other than the skeleton appears to be negligible .
	manualset3
227867	4	421235	7	NULL	NULL	0	NULL	intestine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal young rats , 0.05-0 .1 % of ingested aluminium is absorbed in the intestine , of which roughly half goes to the skeleton within 2 h , whereas the remaining half is excreted in the urine , most of it within 48 h. Deposition in organs other than the skeleton appears to be negligible .
	manualset3
227868	5	421235	7	NULL	NULL	0	NULL	skeleton	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal young rats , 0.05-0 .1 % of ingested aluminium is absorbed in the intestine , of which roughly half goes to the skeleton within 2 h , whereas the remaining half is excreted in the urine , most of it within 48 h. Deposition in organs other than the skeleton appears to be negligible .
	manualset3
227869	6	421235	7	NULL	NULL	0	NULL	2 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal young rats , 0.05-0 .1 % of ingested aluminium is absorbed in the intestine , of which roughly half goes to the skeleton within 2 h , whereas the remaining half is excreted in the urine , most of it within 48 h. Deposition in organs other than the skeleton appears to be negligible .
	manualset3
227870	7	421235	7	NULL	NULL	0	NULL	 urine 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal young rats , 0.05-0 .1 % of ingested aluminium is absorbed in the intestine , of which roughly half goes to the skeleton within 2 h , whereas the remaining half is excreted in the urine , most of it within 48 h. Deposition in organs other than the skeleton appears to be negligible .
	manualset3
227871	8	421235	7	NULL	NULL	0	NULL	48 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal young rats , 0.05-0 .1 % of ingested aluminium is absorbed in the intestine , of which roughly half goes to the skeleton within 2 h , whereas the remaining half is excreted in the urine , most of it within 48 h. Deposition in organs other than the skeleton appears to be negligible .
	manualset3
227872	9	421235	7	NULL	NULL	0	NULL	Deposition 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal young rats , 0.05-0 .1 % of ingested aluminium is absorbed in the intestine , of which roughly half goes to the skeleton within 2 h , whereas the remaining half is excreted in the urine , most of it within 48 h. Deposition in organs other than the skeleton appears to be negligible .
	manualset3
227873	10	421235	7	NULL	NULL	0	NULL	 organs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal young rats , 0.05-0 .1 % of ingested aluminium is absorbed in the intestine , of which roughly half goes to the skeleton within 2 h , whereas the remaining half is excreted in the urine , most of it within 48 h. Deposition in organs other than the skeleton appears to be negligible .
	manualset3
227874	11	421235	7	NULL	NULL	0	NULL	skeleton	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In normal young rats , 0.05-0 .1 % of ingested aluminium is absorbed in the intestine , of which roughly half goes to the skeleton within 2 h , whereas the remaining half is excreted in the urine , most of it within 48 h. Deposition in organs other than the skeleton appears to be negligible .
	manualset3
227875	1	421236	7	NULL	NULL	0	NULL	IRFI-016 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IRFI-016 , a new radical scavenger , limits ischemic damage following coronary artery occlusion in rats .
	manualset3
227876	2	421236	7	NULL	NULL	0	NULL	radical scavenger	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	IRFI-016 , a new radical scavenger , limits ischemic damage following coronary artery occlusion in rats .
	manualset3
227877	3	421236	7	NULL	NULL	0	NULL	ischemic damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	IRFI-016 , a new radical scavenger , limits ischemic damage following coronary artery occlusion in rats .
	manualset3
227878	4	421236	7	NULL	NULL	0	NULL	coronary artery occlusion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IRFI-016 , a new radical scavenger , limits ischemic damage following coronary artery occlusion in rats .
	manualset3
227879	5	421236	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	IRFI-016 , a new radical scavenger , limits ischemic damage following coronary artery occlusion in rats .
	manualset3
227880	1	421237	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data reinforce our hypothesis that a high level of expression of ecNOS in microvessels in the tumor-adjacent area protects against tumor metastasis .
	manualset3
227881	2	421237	7	NULL	NULL	0	NULL	hypothesis 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These data reinforce our hypothesis that a high level of expression of ecNOS in microvessels in the tumor-adjacent area protects against tumor metastasis .
	manualset3
227882	3	421237	7	NULL	NULL	0	NULL	high level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data reinforce our hypothesis that a high level of expression of ecNOS in microvessels in the tumor-adjacent area protects against tumor metastasis .
	manualset3
227883	4	421237	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data reinforce our hypothesis that a high level of expression of ecNOS in microvessels in the tumor-adjacent area protects against tumor metastasis .
	manualset3
227884	5	421237	7	NULL	NULL	0	NULL	ecNOS	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These data reinforce our hypothesis that a high level of expression of ecNOS in microvessels in the tumor-adjacent area protects against tumor metastasis .
	manualset3
227885	6	421237	7	NULL	NULL	0	NULL	microvessels	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	These data reinforce our hypothesis that a high level of expression of ecNOS in microvessels in the tumor-adjacent area protects against tumor metastasis .
	manualset3
227886	7	421237	7	NULL	NULL	0	NULL	tumor-adjacent area	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These data reinforce our hypothesis that a high level of expression of ecNOS in microvessels in the tumor-adjacent area protects against tumor metastasis .
	manualset3
227887	8	421237	7	NULL	NULL	0	NULL	tumor metastasis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data reinforce our hypothesis that a high level of expression of ecNOS in microvessels in the tumor-adjacent area protects against tumor metastasis .
	manualset3
227888	1	421238	7	NULL	NULL	0	NULL	continuous intracarotid injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Under continuous intracarotid injection of 81mKr , the radio activity obtained from the surface of the skull is proportional to the cerebral blood flow .
	manualset3
227889	2	421238	7	NULL	NULL	0	NULL	 81mKr	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Under continuous intracarotid injection of 81mKr , the radio activity obtained from the surface of the skull is proportional to the cerebral blood flow .
	manualset3
227890	3	421238	7	NULL	NULL	0	NULL	radio activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Under continuous intracarotid injection of 81mKr , the radio activity obtained from the surface of the skull is proportional to the cerebral blood flow .
	manualset3
227891	4	421238	7	NULL	NULL	NULL	NULL	surface of the skull	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Under continuous intracarotid injection of 81mKr , the radio activity obtained from the surface of the skull is proportional to the cerebral blood flow .
	manualset3
227893	6	421238	7	NULL	NULL	0	NULL	cerebral blood flow	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Under continuous intracarotid injection of 81mKr , the radio activity obtained from the surface of the skull is proportional to the cerebral blood flow .
	manualset3
227894	1	421239	7	NULL	NULL	0	NULL	Techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Techniques for predicting the lifetimes of wave-swept macroalgae : a primer on fracture mechanics and crack growth .
	manualset3
227895	2	421239	7	NULL	NULL	0	NULL	 lifetimes	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Techniques for predicting the lifetimes of wave-swept macroalgae : a primer on fracture mechanics and crack growth .
	manualset3
227896	3	421239	7	NULL	NULL	0	NULL	wave-swept macroalgae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Techniques for predicting the lifetimes of wave-swept macroalgae : a primer on fracture mechanics and crack growth .
	manualset3
227897	4	421239	7	NULL	NULL	0	NULL	primer	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Techniques for predicting the lifetimes of wave-swept macroalgae : a primer on fracture mechanics and crack growth .
	manualset3
227898	5	421239	7	NULL	NULL	0	NULL	 fracture mechanics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Techniques for predicting the lifetimes of wave-swept macroalgae : a primer on fracture mechanics and crack growth .
	manualset3
227899	6	421239	7	NULL	NULL	0	NULL	crack growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Techniques for predicting the lifetimes of wave-swept macroalgae : a primer on fracture mechanics and crack growth .
	manualset3
227900	1	421240	7	NULL	NULL	0	NULL	enzymatic methods	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Some enzymatic methods are described allowing the quantitation of chemical additives in blood derivatives .
	manualset3
227901	2	421240	7	NULL	NULL	0	NULL	quantitation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Some enzymatic methods are described allowing the quantitation of chemical additives in blood derivatives .
	manualset3
227902	3	421240	7	NULL	NULL	0	NULL	chemical additives 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Some enzymatic methods are described allowing the quantitation of chemical additives in blood derivatives .
	manualset3
227903	4	421240	7	NULL	NULL	0	NULL	blood derivatives	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Some enzymatic methods are described allowing the quantitation of chemical additives in blood derivatives .
	manualset3
227904	1	421241	7	NULL	NULL	0	NULL	case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In each case , the effect of hypophysectomy exceeded that of pituitary stalk transection .
	manualset3
227905	2	421241	7	NULL	NULL	0	NULL	 effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In each case , the effect of hypophysectomy exceeded that of pituitary stalk transection .
	manualset3
227906	3	421241	7	NULL	NULL	0	NULL	hypophysectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In each case , the effect of hypophysectomy exceeded that of pituitary stalk transection .
	manualset3
227907	4	421241	7	NULL	NULL	0	NULL	pituitary stalk transection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In each case , the effect of hypophysectomy exceeded that of pituitary stalk transection .
	manualset3
227908	1	421242	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Further studies on Polypoxvirus chironomi , an insect virus of the pox group isolated from the midge Chironomus luridus .
	manualset3
227909	2	421242	7	NULL	NULL	0	NULL	Polypoxvirus chironomi	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Further studies on Polypoxvirus chironomi , an insect virus of the pox group isolated from the midge Chironomus luridus .
	manualset3
227910	3	421242	7	NULL	NULL	0	NULL	insect virus 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Further studies on Polypoxvirus chironomi , an insect virus of the pox group isolated from the midge Chironomus luridus .
	manualset3
227911	4	421242	7	NULL	NULL	0	NULL	pox group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Further studies on Polypoxvirus chironomi , an insect virus of the pox group isolated from the midge Chironomus luridus .
	manualset3
227912	5	421242	7	NULL	NULL	0	NULL	midge Chironomus luridus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Further studies on Polypoxvirus chironomi , an insect virus of the pox group isolated from the midge Chironomus luridus .
	manualset3
227913	1	421243	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of Paget 's disease of bone by radiotherapy .
	manualset3
227914	2	421243	7	NULL	NULL	0	NULL	Paget 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of Paget 's disease of bone by radiotherapy .
	manualset3
227915	3	421243	7	NULL	NULL	0	NULL	bone 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of Paget 's disease of bone by radiotherapy .
	manualset3
227916	4	421243	7	NULL	NULL	0	NULL	radiotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The treatment of Paget 's disease of bone by radiotherapy .
	manualset3
227917	1	421244	7	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we characterize the metabolic correlates of fat in the liver in a large community-based sample with and without respect to visceral fat .
	manualset3
227918	2	421244	7	NULL	NULL	0	NULL	metabolic correlates	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we characterize the metabolic correlates of fat in the liver in a large community-based sample with and without respect to visceral fat .
	manualset3
227919	3	421244	7	NULL	NULL	0	NULL	fat	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we characterize the metabolic correlates of fat in the liver in a large community-based sample with and without respect to visceral fat .
	manualset3
227920	4	421244	7	NULL	NULL	0	NULL	liver 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we characterize the metabolic correlates of fat in the liver in a large community-based sample with and without respect to visceral fat .
	manualset3
227921	5	421244	7	NULL	NULL	0	NULL	community-based sample	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we characterize the metabolic correlates of fat in the liver in a large community-based sample with and without respect to visceral fat .
	manualset3
227922	6	421244	7	NULL	NULL	0	NULL	 visceral fat 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , we characterize the metabolic correlates of fat in the liver in a large community-based sample with and without respect to visceral fat .
	manualset3
227923	1	421245	7	NULL	NULL	0	NULL	echocardiographic left ventricular mass	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , echocardiographic left ventricular mass normalized for height to the power of the allometric or growth relation between ventricular mass and height was compared in 164 normotensive subjects ( 85 men ( 24 obese ) and 79 women ( 28 obese ) , aged 45 + / - 12 years ) and 475 hypertensive patients ( 325 men ( 126 obese ) and 150 women ( 85 obese ) , aged 54 + / - 10 years ) from an adult employed population .
	manualset3
227924	2	421245	7	NULL	NULL	0	NULL	height	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , echocardiographic left ventricular mass normalized for height to the power of the allometric or growth relation between ventricular mass and height was compared in 164 normotensive subjects ( 85 men ( 24 obese ) and 79 women ( 28 obese ) , aged 45 + / - 12 years ) and 475 hypertensive patients ( 325 men ( 126 obese ) and 150 women ( 85 obese ) , aged 54 + / - 10 years ) from an adult employed population .
	manualset3
227925	3	421245	7	NULL	NULL	0	NULL	power	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , echocardiographic left ventricular mass normalized for height to the power of the allometric or growth relation between ventricular mass and height was compared in 164 normotensive subjects ( 85 men ( 24 obese ) and 79 women ( 28 obese ) , aged 45 + / - 12 years ) and 475 hypertensive patients ( 325 men ( 126 obese ) and 150 women ( 85 obese ) , aged 54 + / - 10 years ) from an adult employed population .
	manualset3
227926	4	421245	7	NULL	NULL	0	NULL	allometric relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , echocardiographic left ventricular mass normalized for height to the power of the allometric or growth relation between ventricular mass and height was compared in 164 normotensive subjects ( 85 men ( 24 obese ) and 79 women ( 28 obese ) , aged 45 + / - 12 years ) and 475 hypertensive patients ( 325 men ( 126 obese ) and 150 women ( 85 obese ) , aged 54 + / - 10 years ) from an adult employed population .
	manualset3
227927	5	421245	7	NULL	NULL	0	NULL	growth relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , echocardiographic left ventricular mass normalized for height to the power of the allometric or growth relation between ventricular mass and height was compared in 164 normotensive subjects ( 85 men ( 24 obese ) and 79 women ( 28 obese ) , aged 45 + / - 12 years ) and 475 hypertensive patients ( 325 men ( 126 obese ) and 150 women ( 85 obese ) , aged 54 + / - 10 years ) from an adult employed population .
	manualset3
227928	6	421245	7	NULL	NULL	0	NULL	ventricular mass	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , echocardiographic left ventricular mass normalized for height to the power of the allometric or growth relation between ventricular mass and height was compared in 164 normotensive subjects ( 85 men ( 24 obese ) and 79 women ( 28 obese ) , aged 45 + / - 12 years ) and 475 hypertensive patients ( 325 men ( 126 obese ) and 150 women ( 85 obese ) , aged 54 + / - 10 years ) from an adult employed population .
	manualset3
227929	7	421245	7	NULL	NULL	0	NULL	height 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , echocardiographic left ventricular mass normalized for height to the power of the allometric or growth relation between ventricular mass and height was compared in 164 normotensive subjects ( 85 men ( 24 obese ) and 79 women ( 28 obese ) , aged 45 + / - 12 years ) and 475 hypertensive patients ( 325 men ( 126 obese ) and 150 women ( 85 obese ) , aged 54 + / - 10 years ) from an adult employed population .
	manualset3
227930	8	421245	7	NULL	NULL	0	NULL	164 normotensive subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , echocardiographic left ventricular mass normalized for height to the power of the allometric or growth relation between ventricular mass and height was compared in 164 normotensive subjects ( 85 men ( 24 obese ) and 79 women ( 28 obese ) , aged 45 + / - 12 years ) and 475 hypertensive patients ( 325 men ( 126 obese ) and 150 women ( 85 obese ) , aged 54 + / - 10 years ) from an adult employed population .
	manualset3
227931	9	421245	7	NULL	NULL	0	NULL	85 men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , echocardiographic left ventricular mass normalized for height to the power of the allometric or growth relation between ventricular mass and height was compared in 164 normotensive subjects ( 85 men ( 24 obese ) and 79 women ( 28 obese ) , aged 45 + / - 12 years ) and 475 hypertensive patients ( 325 men ( 126 obese ) and 150 women ( 85 obese ) , aged 54 + / - 10 years ) from an adult employed population .
	manualset3
227932	10	421245	7	NULL	NULL	0	NULL	24 obese	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , echocardiographic left ventricular mass normalized for height to the power of the allometric or growth relation between ventricular mass and height was compared in 164 normotensive subjects ( 85 men ( 24 obese ) and 79 women ( 28 obese ) , aged 45 + / - 12 years ) and 475 hypertensive patients ( 325 men ( 126 obese ) and 150 women ( 85 obese ) , aged 54 + / - 10 years ) from an adult employed population .
	manualset3
227933	11	421245	7	NULL	NULL	0	NULL	79 women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , echocardiographic left ventricular mass normalized for height to the power of the allometric or growth relation between ventricular mass and height was compared in 164 normotensive subjects ( 85 men ( 24 obese ) and 79 women ( 28 obese ) , aged 45 + / - 12 years ) and 475 hypertensive patients ( 325 men ( 126 obese ) and 150 women ( 85 obese ) , aged 54 + / - 10 years ) from an adult employed population .
	manualset3
227934	12	421245	7	NULL	NULL	0	NULL	28 obese	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , echocardiographic left ventricular mass normalized for height to the power of the allometric or growth relation between ventricular mass and height was compared in 164 normotensive subjects ( 85 men ( 24 obese ) and 79 women ( 28 obese ) , aged 45 + / - 12 years ) and 475 hypertensive patients ( 325 men ( 126 obese ) and 150 women ( 85 obese ) , aged 54 + / - 10 years ) from an adult employed population .
	manualset3
227935	13	421245	7	NULL	NULL	0	NULL	aged 45 + / - 12 years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , echocardiographic left ventricular mass normalized for height to the power of the allometric or growth relation between ventricular mass and height was compared in 164 normotensive subjects ( 85 men ( 24 obese ) and 79 women ( 28 obese ) , aged 45 + / - 12 years ) and 475 hypertensive patients ( 325 men ( 126 obese ) and 150 women ( 85 obese ) , aged 54 + / - 10 years ) from an adult employed population .
	manualset3
227936	14	421245	7	NULL	NULL	0	NULL	475 hypertensive patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , echocardiographic left ventricular mass normalized for height to the power of the allometric or growth relation between ventricular mass and height was compared in 164 normotensive subjects ( 85 men ( 24 obese ) and 79 women ( 28 obese ) , aged 45 + / - 12 years ) and 475 hypertensive patients ( 325 men ( 126 obese ) and 150 women ( 85 obese ) , aged 54 + / - 10 years ) from an adult employed population .
	manualset3
227937	15	421245	7	NULL	NULL	0	NULL	325 men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , echocardiographic left ventricular mass normalized for height to the power of the allometric or growth relation between ventricular mass and height was compared in 164 normotensive subjects ( 85 men ( 24 obese ) and 79 women ( 28 obese ) , aged 45 + / - 12 years ) and 475 hypertensive patients ( 325 men ( 126 obese ) and 150 women ( 85 obese ) , aged 54 + / - 10 years ) from an adult employed population .
	manualset3
227938	16	421245	7	NULL	NULL	0	NULL	126 obese	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , echocardiographic left ventricular mass normalized for height to the power of the allometric or growth relation between ventricular mass and height was compared in 164 normotensive subjects ( 85 men ( 24 obese ) and 79 women ( 28 obese ) , aged 45 + / - 12 years ) and 475 hypertensive patients ( 325 men ( 126 obese ) and 150 women ( 85 obese ) , aged 54 + / - 10 years ) from an adult employed population .
	manualset3
227939	17	421245	7	NULL	NULL	0	NULL	150 women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , echocardiographic left ventricular mass normalized for height to the power of the allometric or growth relation between ventricular mass and height was compared in 164 normotensive subjects ( 85 men ( 24 obese ) and 79 women ( 28 obese ) , aged 45 + / - 12 years ) and 475 hypertensive patients ( 325 men ( 126 obese ) and 150 women ( 85 obese ) , aged 54 + / - 10 years ) from an adult employed population .
	manualset3
227940	18	421245	7	NULL	NULL	0	NULL	 85 obese 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , echocardiographic left ventricular mass normalized for height to the power of the allometric or growth relation between ventricular mass and height was compared in 164 normotensive subjects ( 85 men ( 24 obese ) and 79 women ( 28 obese ) , aged 45 + / - 12 years ) and 475 hypertensive patients ( 325 men ( 126 obese ) and 150 women ( 85 obese ) , aged 54 + / - 10 years ) from an adult employed population .
	manualset3
227941	19	421245	7	NULL	NULL	0	NULL	aged 54 + / - 10 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , echocardiographic left ventricular mass normalized for height to the power of the allometric or growth relation between ventricular mass and height was compared in 164 normotensive subjects ( 85 men ( 24 obese ) and 79 women ( 28 obese ) , aged 45 + / - 12 years ) and 475 hypertensive patients ( 325 men ( 126 obese ) and 150 women ( 85 obese ) , aged 54 + / - 10 years ) from an adult employed population .
	manualset3
227942	20	421245	7	NULL	NULL	0	NULL	 adult employed population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , echocardiographic left ventricular mass normalized for height to the power of the allometric or growth relation between ventricular mass and height was compared in 164 normotensive subjects ( 85 men ( 24 obese ) and 79 women ( 28 obese ) , aged 45 + / - 12 years ) and 475 hypertensive patients ( 325 men ( 126 obese ) and 150 women ( 85 obese ) , aged 54 + / - 10 years ) from an adult employed population .
	manualset3
227943	1	421246	7	NULL	NULL	0	NULL	intraocular penetration 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The intraocular penetration of ( 14C ) fosfonet was studied following topical application of 25 mg of an ointment containing 5 % ( 14C ) fosfonet sodium onto the intact and abraded eyes of New Zealand white rabbits .
	manualset3
227944	2	421246	7	NULL	NULL	0	NULL	( 14C ) fosfonet	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The intraocular penetration of ( 14C ) fosfonet was studied following topical application of 25 mg of an ointment containing 5 % ( 14C ) fosfonet sodium onto the intact and abraded eyes of New Zealand white rabbits .
	manualset3
227945	3	421246	7	NULL	NULL	0	NULL	topical application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The intraocular penetration of ( 14C ) fosfonet was studied following topical application of 25 mg of an ointment containing 5 % ( 14C ) fosfonet sodium onto the intact and abraded eyes of New Zealand white rabbits .
	manualset3
227946	4	421246	7	NULL	NULL	0	NULL	25 mg	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The intraocular penetration of ( 14C ) fosfonet was studied following topical application of 25 mg of an ointment containing 5 % ( 14C ) fosfonet sodium onto the intact and abraded eyes of New Zealand white rabbits .
	manualset3
227947	5	421246	7	NULL	NULL	0	NULL	ointment 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The intraocular penetration of ( 14C ) fosfonet was studied following topical application of 25 mg of an ointment containing 5 % ( 14C ) fosfonet sodium onto the intact and abraded eyes of New Zealand white rabbits .
	manualset3
227948	6	421246	7	NULL	NULL	0	NULL	5 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The intraocular penetration of ( 14C ) fosfonet was studied following topical application of 25 mg of an ointment containing 5 % ( 14C ) fosfonet sodium onto the intact and abraded eyes of New Zealand white rabbits .
	manualset3
227949	7	421246	7	NULL	NULL	0	NULL	( 14C ) fosfonet sodium	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The intraocular penetration of ( 14C ) fosfonet was studied following topical application of 25 mg of an ointment containing 5 % ( 14C ) fosfonet sodium onto the intact and abraded eyes of New Zealand white rabbits .
	manualset3
227950	8	421246	7	NULL	NULL	0	NULL	abraded eyes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The intraocular penetration of ( 14C ) fosfonet was studied following topical application of 25 mg of an ointment containing 5 % ( 14C ) fosfonet sodium onto the intact and abraded eyes of New Zealand white rabbits .
	manualset3
227951	9	421246	7	NULL	NULL	0	NULL	New Zealand white rabbits	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The intraocular penetration of ( 14C ) fosfonet was studied following topical application of 25 mg of an ointment containing 5 % ( 14C ) fosfonet sodium onto the intact and abraded eyes of New Zealand white rabbits .
	manualset3
227952	1	421247	7	NULL	NULL	0	NULL	control patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All the control patients remain seropositive for HBsAg , HBeAg and DNA polymerase activity .
	manualset3
227954	3	421247	7	NULL	NULL	0	NULL	HBsAg activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All the control patients remain seropositive for HBsAg , HBeAg and DNA polymerase activity .
	manualset3
227955	4	421247	7	NULL	NULL	0	NULL	HBeAg activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All the control patients remain seropositive for HBsAg , HBeAg and DNA polymerase activity .
	manualset3
227956	5	421247	7	NULL	NULL	0	NULL	DNA polymerase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All the control patients remain seropositive for HBsAg , HBeAg and DNA polymerase activity .
	manualset3
227957	1	421248	7	NULL	NULL	0	NULL	Fifty percent	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Fifty percent of the sample could correctly define the term infant mortality .
	manualset3
227958	2	421248	7	NULL	NULL	0	NULL	sample	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Fifty percent of the sample could correctly define the term infant mortality .
	manualset3
227959	3	421248	7	NULL	NULL	0	NULL	term	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Fifty percent of the sample could correctly define the term infant mortality .
	manualset3
227960	4	421248	7	NULL	NULL	0	NULL	infant mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Fifty percent of the sample could correctly define the term infant mortality .
	manualset3
227961	1	421249	7	NULL	NULL	0	NULL	Soy isoflavones	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Soy isoflavones exert inconsistent bone density-preserving effects , but the bone strength-preserving effects in humans are unknown .
	manualset3
227962	2	421249	7	NULL	NULL	0	NULL	inconsistent bone density-preserving effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Soy isoflavones exert inconsistent bone density-preserving effects , but the bone strength-preserving effects in humans are unknown .
	manualset3
227963	3	421249	7	NULL	NULL	NULL	NULL	bone strength-preserving effects	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Soy isoflavones exert inconsistent bone density-preserving effects , but the bone strength-preserving effects in humans are unknown .
	manualset3
227964	4	421249	7	NULL	NULL	0	NULL	humans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Soy isoflavones exert inconsistent bone density-preserving effects , but the bone strength-preserving effects in humans are unknown .
	manualset3
227965	1	421250	7	NULL	NULL	0	NULL	 basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of their results , the authors conclude that the lysosomal damage caused by CCl4 is mediated by peroxidation of lipids and the lysosomal membrane can be stabilised by MTDQ .
	manualset3
227966	2	421250	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of their results , the authors conclude that the lysosomal damage caused by CCl4 is mediated by peroxidation of lipids and the lysosomal membrane can be stabilised by MTDQ .
	manualset3
227967	3	421250	7	NULL	NULL	0	NULL	authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of their results , the authors conclude that the lysosomal damage caused by CCl4 is mediated by peroxidation of lipids and the lysosomal membrane can be stabilised by MTDQ .
	manualset3
227968	4	421250	7	NULL	NULL	0	NULL	lysosomal damage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of their results , the authors conclude that the lysosomal damage caused by CCl4 is mediated by peroxidation of lipids and the lysosomal membrane can be stabilised by MTDQ .
	manualset3
227969	5	421250	7	NULL	NULL	0	NULL	CCl4	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of their results , the authors conclude that the lysosomal damage caused by CCl4 is mediated by peroxidation of lipids and the lysosomal membrane can be stabilised by MTDQ .
	manualset3
227970	6	421250	7	NULL	NULL	0	NULL	peroxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of their results , the authors conclude that the lysosomal damage caused by CCl4 is mediated by peroxidation of lipids and the lysosomal membrane can be stabilised by MTDQ .
	manualset3
227971	7	421250	7	NULL	NULL	0	NULL	lipids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of their results , the authors conclude that the lysosomal damage caused by CCl4 is mediated by peroxidation of lipids and the lysosomal membrane can be stabilised by MTDQ .
	manualset3
227972	8	421250	7	NULL	NULL	0	NULL	 lysosomal membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of their results , the authors conclude that the lysosomal damage caused by CCl4 is mediated by peroxidation of lipids and the lysosomal membrane can be stabilised by MTDQ .
	manualset3
227973	9	421250	7	NULL	NULL	0	NULL	MTDQ	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On the basis of their results , the authors conclude that the lysosomal damage caused by CCl4 is mediated by peroxidation of lipids and the lysosomal membrane can be stabilised by MTDQ .
	manualset3
227974	1	421251	7	NULL	NULL	0	NULL	no patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In no patient were the results of lidocaine and steroid injection superior to botulinum chemodenervation .
	manualset3
227975	2	421251	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In no patient were the results of lidocaine and steroid injection superior to botulinum chemodenervation .
	manualset3
227976	3	421251	7	NULL	NULL	0	NULL	lidocaine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In no patient were the results of lidocaine and steroid injection superior to botulinum chemodenervation .
	manualset3
227977	4	421251	7	NULL	NULL	0	NULL	steroid injection 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In no patient were the results of lidocaine and steroid injection superior to botulinum chemodenervation .
	manualset3
227978	5	421251	7	NULL	NULL	0	NULL	botulinum chemodenervation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In no patient were the results of lidocaine and steroid injection superior to botulinum chemodenervation .
	manualset3
227979	1	421252	7	NULL	NULL	0	NULL	Amyloidosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Amyloidosis could be one factor inducing the fowlpox infection in vaccinated chickens .
	manualset3
227980	2	421252	7	NULL	NULL	NULL	NULL	one factor	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Amyloidosis could be one factor inducing the fowlpox infection in vaccinated chickens .
	manualset3
227981	3	421252	7	NULL	NULL	0	NULL	fowlpox infection	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Amyloidosis could be one factor inducing the fowlpox infection in vaccinated chickens .
	manualset3
227982	4	421252	7	NULL	NULL	0	NULL	vaccinated chickens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Amyloidosis could be one factor inducing the fowlpox infection in vaccinated chickens .
	manualset3
227983	1	421253	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with cyclophosphamide ( Cy ) before contact sensitization regularly intensifies the induced sensitivity .
	manualset3
227984	2	421253	7	NULL	NULL	0	NULL	cyclophosphamide ( Cy )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with cyclophosphamide ( Cy ) before contact sensitization regularly intensifies the induced sensitivity .
	manualset3
227985	3	421253	7	NULL	NULL	0	NULL	 contact sensitization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with cyclophosphamide ( Cy ) before contact sensitization regularly intensifies the induced sensitivity .
	manualset3
227986	4	421253	7	NULL	NULL	0	NULL	 induced sensitivity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with cyclophosphamide ( Cy ) before contact sensitization regularly intensifies the induced sensitivity .
	manualset3
227987	1	421254	7	NULL	NULL	0	NULL	Immunoreactive aconitase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoreactive aconitase was also low .
	manualset3
227988	1	421255	7	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , our data reveal that Smarcc1 plays important roles in facilitating mESCs differentiation by coupling gene repression with global and local changes in chromatin structure .
	manualset3
227989	2	421255	7	NULL	NULL	0	NULL	Smarcc1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , our data reveal that Smarcc1 plays important roles in facilitating mESCs differentiation by coupling gene repression with global and local changes in chromatin structure .
	manualset3
227990	3	421255	7	NULL	NULL	0	NULL	important roles	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , our data reveal that Smarcc1 plays important roles in facilitating mESCs differentiation by coupling gene repression with global and local changes in chromatin structure .
	manualset3
227991	4	421255	7	NULL	NULL	0	NULL	mESCs differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , our data reveal that Smarcc1 plays important roles in facilitating mESCs differentiation by coupling gene repression with global and local changes in chromatin structure .
	manualset3
227992	5	421255	7	NULL	NULL	0	NULL	gene repression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , our data reveal that Smarcc1 plays important roles in facilitating mESCs differentiation by coupling gene repression with global and local changes in chromatin structure .
	manualset3
227993	6	421255	7	NULL	NULL	0	NULL	global changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , our data reveal that Smarcc1 plays important roles in facilitating mESCs differentiation by coupling gene repression with global and local changes in chromatin structure .
	manualset3
227994	7	421255	7	NULL	NULL	0	NULL	local changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , our data reveal that Smarcc1 plays important roles in facilitating mESCs differentiation by coupling gene repression with global and local changes in chromatin structure .
	manualset3
227995	8	421255	7	NULL	NULL	NULL	NULL	chromatin structure	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Collectively , our data reveal that Smarcc1 plays important roles in facilitating mESCs differentiation by coupling gene repression with global and local changes in chromatin structure .
	manualset3
227996	1	421256	7	NULL	NULL	0	NULL	 cryotherapy treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , cryotherapy treatment , including cryotherapy managed by nurses immediately after screening , was well-received by women in the studies .
	manualset3
227997	2	421256	7	NULL	NULL	0	NULL	cryotherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , cryotherapy treatment , including cryotherapy managed by nurses immediately after screening , was well-received by women in the studies .
	manualset3
227998	3	421256	7	NULL	NULL	0	NULL	nurses	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , cryotherapy treatment , including cryotherapy managed by nurses immediately after screening , was well-received by women in the studies .
	manualset3
227999	4	421256	7	NULL	NULL	0	NULL	 screening	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , cryotherapy treatment , including cryotherapy managed by nurses immediately after screening , was well-received by women in the studies .
	manualset3
228000	5	421256	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , cryotherapy treatment , including cryotherapy managed by nurses immediately after screening , was well-received by women in the studies .
	manualset3
228001	6	421256	7	NULL	NULL	0	NULL	 studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Similarly , cryotherapy treatment , including cryotherapy managed by nurses immediately after screening , was well-received by women in the studies .
	manualset3
228002	1	421257	7	NULL	NULL	0	NULL	Coomooboolaroo , Qld	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	At Coomooboolaroo , Qld , the X chromosome was also a large submetacentric but a secondary constriction occurred in the shorter arm .
	manualset3
228003	2	421257	7	NULL	NULL	0	NULL	X chromosome	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	At Coomooboolaroo , Qld , the X chromosome was also a large submetacentric but a secondary constriction occurred in the shorter arm .
	manualset3
228004	3	421257	7	NULL	NULL	0	NULL	large submetacentric	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	At Coomooboolaroo , Qld , the X chromosome was also a large submetacentric but a secondary constriction occurred in the shorter arm .
	manualset3
228005	4	421257	7	NULL	NULL	0	NULL	 secondary constriction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	At Coomooboolaroo , Qld , the X chromosome was also a large submetacentric but a secondary constriction occurred in the shorter arm .
	manualset3
228006	5	421257	7	NULL	NULL	0	NULL	shorter arm	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	At Coomooboolaroo , Qld , the X chromosome was also a large submetacentric but a secondary constriction occurred in the shorter arm .
	manualset3
228007	1	421258	7	NULL	NULL	0	NULL	SP-induced scratching	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	SP-induced scratching was inhibited by the NK1 receptor antagonists spantide and L-668 , 169 , but not by the NK2 antagonist L-659 , 877 .
	manualset3
228008	2	421258	7	NULL	NULL	0	NULL	NK1 receptor antagonists	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	SP-induced scratching was inhibited by the NK1 receptor antagonists spantide and L-668 , 169 , but not by the NK2 antagonist L-659 , 877 .
	manualset3
228009	3	421258	7	NULL	NULL	0	NULL	spantide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	SP-induced scratching was inhibited by the NK1 receptor antagonists spantide and L-668 , 169 , but not by the NK2 antagonist L-659 , 877 .
	manualset3
228010	4	421258	7	NULL	NULL	0	NULL	L-668	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	SP-induced scratching was inhibited by the NK1 receptor antagonists spantide and L-668 , 169 , but not by the NK2 antagonist L-659 , 877 .
	manualset3
228011	5	421258	7	NULL	NULL	0	NULL	L-169	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	SP-induced scratching was inhibited by the NK1 receptor antagonists spantide and L-668 , 169 , but not by the NK2 antagonist L-659 , 877 .
	manualset3
228012	6	421258	7	NULL	NULL	0	NULL	NK2 antagonist	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	SP-induced scratching was inhibited by the NK1 receptor antagonists spantide and L-668 , 169 , but not by the NK2 antagonist L-659 , 877 .
	manualset3
228013	7	421258	7	NULL	NULL	0	NULL	 L-659	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	SP-induced scratching was inhibited by the NK1 receptor antagonists spantide and L-668 , 169 , but not by the NK2 antagonist L-659 , 877 .
	manualset3
228014	8	421258	7	NULL	NULL	0	NULL	L-877	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	SP-induced scratching was inhibited by the NK1 receptor antagonists spantide and L-668 , 169 , but not by the NK2 antagonist L-659 , 877 .
	manualset3
228015	1	421259	7	NULL	NULL	0	NULL	Optical tools	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Optical tools may increase the survey especially in short incisions .
	manualset3
228016	2	421259	7	NULL	NULL	0	NULL	survey	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Optical tools may increase the survey especially in short incisions .
	manualset3
228017	3	421259	7	NULL	NULL	0	NULL	short incisions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Optical tools may increase the survey especially in short incisions .
	manualset3
228018	1	421260	7	NULL	NULL	0	NULL	Conclusions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : As compared with SES and PES , the use of ZES in patients with STEMI undergoing primary PCI , showed similar rates of MACE , cardiac death and recurrent MI at 12 and 18 months .
	manualset3
228019	2	421260	7	NULL	NULL	0	NULL	SES	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : As compared with SES and PES , the use of ZES in patients with STEMI undergoing primary PCI , showed similar rates of MACE , cardiac death and recurrent MI at 12 and 18 months .
	manualset3
228020	3	421260	7	NULL	NULL	0	NULL	PES	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : As compared with SES and PES , the use of ZES in patients with STEMI undergoing primary PCI , showed similar rates of MACE , cardiac death and recurrent MI at 12 and 18 months .
	manualset3
228021	4	421260	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : As compared with SES and PES , the use of ZES in patients with STEMI undergoing primary PCI , showed similar rates of MACE , cardiac death and recurrent MI at 12 and 18 months .
	manualset3
228022	5	421260	7	NULL	NULL	0	NULL	ZES	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : As compared with SES and PES , the use of ZES in patients with STEMI undergoing primary PCI , showed similar rates of MACE , cardiac death and recurrent MI at 12 and 18 months .
	manualset3
228023	6	421260	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : As compared with SES and PES , the use of ZES in patients with STEMI undergoing primary PCI , showed similar rates of MACE , cardiac death and recurrent MI at 12 and 18 months .
	manualset3
228024	7	421260	7	NULL	NULL	0	NULL	 STEMI	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : As compared with SES and PES , the use of ZES in patients with STEMI undergoing primary PCI , showed similar rates of MACE , cardiac death and recurrent MI at 12 and 18 months .
	manualset3
228025	8	421260	7	NULL	NULL	NULL	NULL	primary PCI	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Conclusions : As compared with SES and PES , the use of ZES in patients with STEMI undergoing primary PCI , showed similar rates of MACE , cardiac death and recurrent MI at 12 and 18 months .
	manualset3
228026	9	421260	7	NULL	NULL	0	NULL	 similar rates 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : As compared with SES and PES , the use of ZES in patients with STEMI undergoing primary PCI , showed similar rates of MACE , cardiac death and recurrent MI at 12 and 18 months .
	manualset3
228027	10	421260	7	NULL	NULL	0	NULL	MACE	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : As compared with SES and PES , the use of ZES in patients with STEMI undergoing primary PCI , showed similar rates of MACE , cardiac death and recurrent MI at 12 and 18 months .
	manualset3
228028	11	421260	7	NULL	NULL	0	NULL	cardiac death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : As compared with SES and PES , the use of ZES in patients with STEMI undergoing primary PCI , showed similar rates of MACE , cardiac death and recurrent MI at 12 and 18 months .
	manualset3
228029	12	421260	7	NULL	NULL	0	NULL	 recurrent MI	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : As compared with SES and PES , the use of ZES in patients with STEMI undergoing primary PCI , showed similar rates of MACE , cardiac death and recurrent MI at 12 and 18 months .
	manualset3
228030	13	421260	7	NULL	NULL	0	NULL	 12 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : As compared with SES and PES , the use of ZES in patients with STEMI undergoing primary PCI , showed similar rates of MACE , cardiac death and recurrent MI at 12 and 18 months .
	manualset3
228031	14	421260	7	NULL	NULL	0	NULL	18 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : As compared with SES and PES , the use of ZES in patients with STEMI undergoing primary PCI , showed similar rates of MACE , cardiac death and recurrent MI at 12 and 18 months .
	manualset3
228136	1	421261	7	NULL	NULL	0	NULL	Sections	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Sections of the uteri of 10 patients who had used IUDs for several months to 2 years were stained and treated by microchemical techniques to determine DNS , PNS , and copper levels .
	manualset3
228137	2	421261	7	NULL	NULL	0	NULL	 uteri 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Sections of the uteri of 10 patients who had used IUDs for several months to 2 years were stained and treated by microchemical techniques to determine DNS , PNS , and copper levels .
	manualset3
228138	3	421261	7	NULL	NULL	0	NULL	10 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sections of the uteri of 10 patients who had used IUDs for several months to 2 years were stained and treated by microchemical techniques to determine DNS , PNS , and copper levels .
	manualset3
228139	4	421261	7	NULL	NULL	0	NULL	IUDs	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Sections of the uteri of 10 patients who had used IUDs for several months to 2 years were stained and treated by microchemical techniques to determine DNS , PNS , and copper levels .
	manualset3
228140	5	421261	7	NULL	NULL	0	NULL	 several months 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Sections of the uteri of 10 patients who had used IUDs for several months to 2 years were stained and treated by microchemical techniques to determine DNS , PNS , and copper levels .
	manualset3
228141	6	421261	7	NULL	NULL	0	NULL	 2 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Sections of the uteri of 10 patients who had used IUDs for several months to 2 years were stained and treated by microchemical techniques to determine DNS , PNS , and copper levels .
	manualset3
228142	7	421261	7	NULL	NULL	0	NULL	microchemical techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sections of the uteri of 10 patients who had used IUDs for several months to 2 years were stained and treated by microchemical techniques to determine DNS , PNS , and copper levels .
	manualset3
228143	8	421261	7	NULL	NULL	0	NULL	DNS levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sections of the uteri of 10 patients who had used IUDs for several months to 2 years were stained and treated by microchemical techniques to determine DNS , PNS , and copper levels .
	manualset3
228144	9	421261	7	NULL	NULL	0	NULL	PNS levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sections of the uteri of 10 patients who had used IUDs for several months to 2 years were stained and treated by microchemical techniques to determine DNS , PNS , and copper levels .
	manualset3
228145	10	421261	7	NULL	NULL	0	NULL	copper levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sections of the uteri of 10 patients who had used IUDs for several months to 2 years were stained and treated by microchemical techniques to determine DNS , PNS , and copper levels .
	manualset3
228146	1	421262	7	NULL	NULL	0	NULL	Amylose	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Amylose formed helical inclusion complexes with the fatty acid .
	manualset3
228147	2	421262	7	NULL	NULL	0	NULL	 helical inclusion complexes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Amylose formed helical inclusion complexes with the fatty acid .
	manualset3
228149	3	421262	7	NULL	NULL	0	NULL	fatty acid	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Amylose formed helical inclusion complexes with the fatty acid .
	manualset3
228150	1	421263	7	NULL	NULL	0	NULL	Protein engineering efforts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein engineering efforts to design optimal thrombolytics will likely be affected by the permeation processes that occur during thrombolysis .
	manualset3
228152	2	421263	7	NULL	NULL	0	NULL	optimal thrombolytics	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein engineering efforts to design optimal thrombolytics will likely be affected by the permeation processes that occur during thrombolysis .
	manualset3
228154	3	421263	7	NULL	NULL	0	NULL	permeation processes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein engineering efforts to design optimal thrombolytics will likely be affected by the permeation processes that occur during thrombolysis .
	manualset3
228155	4	421263	7	NULL	NULL	0	NULL	thrombolysis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein engineering efforts to design optimal thrombolytics will likely be affected by the permeation processes that occur during thrombolysis .
	manualset3
228157	1	421264	7	NULL	NULL	0	NULL	4 cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 4 cases ( 7 % ) the plaques were hypoechoic and corresponded to a localized widening of the pericavernous tissues : this condition was observed more frequently in the earliest stages of the disease .
	manualset3
228158	2	421264	7	NULL	NULL	0	NULL	7 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 4 cases ( 7 % ) the plaques were hypoechoic and corresponded to a localized widening of the pericavernous tissues : this condition was observed more frequently in the earliest stages of the disease .
	manualset3
228159	3	421264	7	NULL	NULL	0	NULL	 plaques	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 4 cases ( 7 % ) the plaques were hypoechoic and corresponded to a localized widening of the pericavernous tissues : this condition was observed more frequently in the earliest stages of the disease .
	manualset3
228160	4	421264	7	NULL	NULL	0	NULL	 localized widening	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In 4 cases ( 7 % ) the plaques were hypoechoic and corresponded to a localized widening of the pericavernous tissues : this condition was observed more frequently in the earliest stages of the disease .
	manualset3
228161	5	421264	7	NULL	NULL	0	NULL	pericavernous tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In 4 cases ( 7 % ) the plaques were hypoechoic and corresponded to a localized widening of the pericavernous tissues : this condition was observed more frequently in the earliest stages of the disease .
	manualset3
228162	6	421264	7	NULL	NULL	0	NULL	condition 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 4 cases ( 7 % ) the plaques were hypoechoic and corresponded to a localized widening of the pericavernous tissues : this condition was observed more frequently in the earliest stages of the disease .
	manualset3
228164	7	421264	7	NULL	NULL	0	NULL	earliest stages 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In 4 cases ( 7 % ) the plaques were hypoechoic and corresponded to a localized widening of the pericavernous tissues : this condition was observed more frequently in the earliest stages of the disease .
	manualset3
228166	8	421264	7	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In 4 cases ( 7 % ) the plaques were hypoechoic and corresponded to a localized widening of the pericavernous tissues : this condition was observed more frequently in the earliest stages of the disease .
	manualset3
228168	1	421265	7	NULL	NULL	0	NULL	CDP-derived hydroxyproline content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been found that CDP-derived hydroxyproline content in aortic aneurysm was increased as compared with normal aorta , suggesting an increased collagen degradation .
	manualset3
228169	2	421265	7	NULL	NULL	0	NULL	aortic aneurysm	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been found that CDP-derived hydroxyproline content in aortic aneurysm was increased as compared with normal aorta , suggesting an increased collagen degradation .
	manualset3
228170	3	421265	7	NULL	NULL	0	NULL	normal aorta	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been found that CDP-derived hydroxyproline content in aortic aneurysm was increased as compared with normal aorta , suggesting an increased collagen degradation .
	manualset3
228171	4	421265	7	NULL	NULL	NULL	NULL	increased collagen degradation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It has been found that CDP-derived hydroxyproline content in aortic aneurysm was increased as compared with normal aorta , suggesting an increased collagen degradation .
	manualset3
228172	1	421266	7	NULL	NULL	0	NULL	latter type	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter type may be involuntary , voluntary or caused by abdominal pressure .
	manualset3
228175	2	421266	7	NULL	NULL	NULL	NULL	abdominal pressure 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The latter type may be involuntary , voluntary or caused by abdominal pressure .
	manualset3
228177	1	421267	7	NULL	NULL	0	NULL	 previous studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the previous studies on the effects of iron deficiency on skeletal muscle respiratory capacity and work performance have been investigated in severe or moderate iron-deficiency anemia .
	manualset3
228178	2	421267	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the previous studies on the effects of iron deficiency on skeletal muscle respiratory capacity and work performance have been investigated in severe or moderate iron-deficiency anemia .
	manualset3
228179	3	421267	7	NULL	NULL	0	NULL	 iron deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the previous studies on the effects of iron deficiency on skeletal muscle respiratory capacity and work performance have been investigated in severe or moderate iron-deficiency anemia .
	manualset3
228180	4	421267	7	NULL	NULL	0	NULL	skeletal muscle respiratory capacity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the previous studies on the effects of iron deficiency on skeletal muscle respiratory capacity and work performance have been investigated in severe or moderate iron-deficiency anemia .
	manualset3
228181	5	421267	7	NULL	NULL	0	NULL	work performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the previous studies on the effects of iron deficiency on skeletal muscle respiratory capacity and work performance have been investigated in severe or moderate iron-deficiency anemia .
	manualset3
228182	6	421267	7	NULL	NULL	0	NULL	moderate iron-deficiency anemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the previous studies on the effects of iron deficiency on skeletal muscle respiratory capacity and work performance have been investigated in severe or moderate iron-deficiency anemia .
	manualset3
228184	7	421267	7	NULL	NULL	0	NULL	severe iron-deficiency anemia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Most of the previous studies on the effects of iron deficiency on skeletal muscle respiratory capacity and work performance have been investigated in severe or moderate iron-deficiency anemia .
	manualset3
228186	1	421268	7	NULL	NULL	0	NULL	high concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A high concentration of PHV , the C-terminally extended form of PHI which includes prepro-VIP 111-122 , was found in the small intestine .
	manualset3
228187	2	421268	7	NULL	NULL	0	NULL	PHV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A high concentration of PHV , the C-terminally extended form of PHI which includes prepro-VIP 111-122 , was found in the small intestine .
	manualset3
228189	3	421268	7	NULL	NULL	0	NULL	C-terminally extended form of PHI	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A high concentration of PHV , the C-terminally extended form of PHI which includes prepro-VIP 111-122 , was found in the small intestine .
	manualset3
228190	4	421268	7	NULL	NULL	0	NULL	 prepro-VIP 111-122	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A high concentration of PHV , the C-terminally extended form of PHI which includes prepro-VIP 111-122 , was found in the small intestine .
	manualset3
228192	5	421268	7	NULL	NULL	0	NULL	small intestine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A high concentration of PHV , the C-terminally extended form of PHI which includes prepro-VIP 111-122 , was found in the small intestine .
	manualset3
228194	1	421269	7	NULL	NULL	0	NULL	Acute Sinusitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute Sinusitis and Technique of the Antrum Washout .
	manualset3
228196	2	421269	7	NULL	NULL	0	NULL	Technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute Sinusitis and Technique of the Antrum Washout .
	manualset3
228197	3	421269	7	NULL	NULL	0	NULL	Antrum Washout	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Acute Sinusitis and Technique of the Antrum Washout .
	manualset3
228199	1	421270	7	NULL	NULL	0	NULL	POI 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	To follow POI , 54 % of EDs use the ED itself , and 59 % send patients to community physicians .
	manualset3
228200	2	421270	7	NULL	NULL	0	NULL	EDs	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	To follow POI , 54 % of EDs use the ED itself , and 59 % send patients to community physicians .
	manualset3
228201	3	421270	7	NULL	NULL	0	NULL	ED 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	To follow POI , 54 % of EDs use the ED itself , and 59 % send patients to community physicians .
	manualset3
228204	4	421270	7	NULL	NULL	0	NULL	59 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To follow POI , 54 % of EDs use the ED itself , and 59 % send patients to community physicians .
	manualset3
228205	5	421270	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To follow POI , 54 % of EDs use the ED itself , and 59 % send patients to community physicians .
	manualset3
228207	6	421270	7	NULL	NULL	0	NULL	community physicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	To follow POI , 54 % of EDs use the ED itself , and 59 % send patients to community physicians .
	manualset3
229411	7	421270	7	NULL	NULL	0	NULL	54%	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To follow POI , 54 % of EDs use the ED itself , and 59 % send patients to community physicians .
	manualset3
228211	1	421271	7	NULL	NULL	0	NULL	Small colon intussusception	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Small colon intussusception is an uncommon cause of signs of abdominal pain and is similar to type-IV rectal prolapse .
	manualset3
228213	2	421271	7	NULL	NULL	0	NULL	uncommon cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Small colon intussusception is an uncommon cause of signs of abdominal pain and is similar to type-IV rectal prolapse .
	manualset3
228214	3	421271	7	NULL	NULL	0	NULL	signs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Small colon intussusception is an uncommon cause of signs of abdominal pain and is similar to type-IV rectal prolapse .
	manualset3
228215	4	421271	7	NULL	NULL	0	NULL	abdominal pain 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Small colon intussusception is an uncommon cause of signs of abdominal pain and is similar to type-IV rectal prolapse .
	manualset3
228216	5	421271	7	NULL	NULL	0	NULL	type-IV rectal prolapse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Small colon intussusception is an uncommon cause of signs of abdominal pain and is similar to type-IV rectal prolapse .
	manualset3
228226	1	421272	7	NULL	NULL	0	NULL	Amyotrophic lateral sclerosis ( ALS )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Amyotrophic lateral sclerosis ( ALS ) is a late-onset progressive degeneration of motor neurons occurring both as a sporadic and a familial disease .
	manualset3
228227	2	421272	7	NULL	NULL	0	NULL	late-onset progressive degeneration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Amyotrophic lateral sclerosis ( ALS ) is a late-onset progressive degeneration of motor neurons occurring both as a sporadic and a familial disease .
	manualset3
228228	3	421272	7	NULL	NULL	0	NULL	motor neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Amyotrophic lateral sclerosis ( ALS ) is a late-onset progressive degeneration of motor neurons occurring both as a sporadic and a familial disease .
	manualset3
228229	4	421272	7	NULL	NULL	0	NULL	sporadic disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Amyotrophic lateral sclerosis ( ALS ) is a late-onset progressive degeneration of motor neurons occurring both as a sporadic and a familial disease .
	manualset3
228230	5	421272	7	NULL	NULL	0	NULL	familial disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Amyotrophic lateral sclerosis ( ALS ) is a late-onset progressive degeneration of motor neurons occurring both as a sporadic and a familial disease .
	manualset3
228231	1	421273	7	NULL	NULL	0	NULL	virion glycoprotein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We conclude that the virion glycoprotein requirements for infection of mammalian neurones are similar to those required for infection of fibroblasts and epithelial cells but that glycoprotein C may enhance infection of neurones .
	manualset3
228232	2	421273	7	NULL	NULL	0	NULL	 infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We conclude that the virion glycoprotein requirements for infection of mammalian neurones are similar to those required for infection of fibroblasts and epithelial cells but that glycoprotein C may enhance infection of neurones .
	manualset3
228233	3	421273	7	NULL	NULL	0	NULL	mammalian neurones	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We conclude that the virion glycoprotein requirements for infection of mammalian neurones are similar to those required for infection of fibroblasts and epithelial cells but that glycoprotein C may enhance infection of neurones .
	manualset3
228234	4	421273	7	NULL	NULL	0	NULL	 infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We conclude that the virion glycoprotein requirements for infection of mammalian neurones are similar to those required for infection of fibroblasts and epithelial cells but that glycoprotein C may enhance infection of neurones .
	manualset3
228235	5	421273	7	NULL	NULL	0	NULL	fibroblasts 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We conclude that the virion glycoprotein requirements for infection of mammalian neurones are similar to those required for infection of fibroblasts and epithelial cells but that glycoprotein C may enhance infection of neurones .
	manualset3
228236	6	421273	7	NULL	NULL	0	NULL	epithelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We conclude that the virion glycoprotein requirements for infection of mammalian neurones are similar to those required for infection of fibroblasts and epithelial cells but that glycoprotein C may enhance infection of neurones .
	manualset3
228237	7	421273	7	NULL	NULL	0	NULL	glycoprotein C 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We conclude that the virion glycoprotein requirements for infection of mammalian neurones are similar to those required for infection of fibroblasts and epithelial cells but that glycoprotein C may enhance infection of neurones .
	manualset3
228238	8	421273	7	NULL	NULL	0	NULL	 infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We conclude that the virion glycoprotein requirements for infection of mammalian neurones are similar to those required for infection of fibroblasts and epithelial cells but that glycoprotein C may enhance infection of neurones .
	manualset3
228239	9	421273	7	NULL	NULL	0	NULL	neurones	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We conclude that the virion glycoprotein requirements for infection of mammalian neurones are similar to those required for infection of fibroblasts and epithelial cells but that glycoprotein C may enhance infection of neurones .
	manualset3
228240	1	421274	7	NULL	NULL	0	NULL	US speeds	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The US speeds of artC from the superficial to deep regions were 1518 + / - 17 ( mean + SD ) , 1532 + / - 26 and 1554 + / - 42 m/s for the US beam parallel to the artC surface , and 1574 + / - 29 , 1621 + / - 34 and 1701 + / - 36 m/s for the beam perpendicular to the artC surface .
	manualset3
228241	2	421274	7	NULL	NULL	0	NULL	artC	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The US speeds of artC from the superficial to deep regions were 1518 + / - 17 ( mean + SD ) , 1532 + / - 26 and 1554 + / - 42 m/s for the US beam parallel to the artC surface , and 1574 + / - 29 , 1621 + / - 34 and 1701 + / - 36 m/s for the beam perpendicular to the artC surface .
	manualset3
228242	3	421274	7	NULL	NULL	0	NULL	superficial region	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The US speeds of artC from the superficial to deep regions were 1518 + / - 17 ( mean + SD ) , 1532 + / - 26 and 1554 + / - 42 m/s for the US beam parallel to the artC surface , and 1574 + / - 29 , 1621 + / - 34 and 1701 + / - 36 m/s for the beam perpendicular to the artC surface .
	manualset3
228243	4	421274	7	NULL	NULL	0	NULL	deep regions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The US speeds of artC from the superficial to deep regions were 1518 + / - 17 ( mean + SD ) , 1532 + / - 26 and 1554 + / - 42 m/s for the US beam parallel to the artC surface , and 1574 + / - 29 , 1621 + / - 34 and 1701 + / - 36 m/s for the beam perpendicular to the artC surface .
	manualset3
228244	5	421274	7	NULL	NULL	0	NULL	1518 + / - 17 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The US speeds of artC from the superficial to deep regions were 1518 + / - 17 ( mean + SD ) , 1532 + / - 26 and 1554 + / - 42 m/s for the US beam parallel to the artC surface , and 1574 + / - 29 , 1621 + / - 34 and 1701 + / - 36 m/s for the beam perpendicular to the artC surface .
	manualset3
228245	6	421274	7	NULL	NULL	0	NULL	 mean + SD	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The US speeds of artC from the superficial to deep regions were 1518 + / - 17 ( mean + SD ) , 1532 + / - 26 and 1554 + / - 42 m/s for the US beam parallel to the artC surface , and 1574 + / - 29 , 1621 + / - 34 and 1701 + / - 36 m/s for the beam perpendicular to the artC surface .
	manualset3
228246	7	421274	7	NULL	NULL	0	NULL	1532 + / - 26	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The US speeds of artC from the superficial to deep regions were 1518 + / - 17 ( mean + SD ) , 1532 + / - 26 and 1554 + / - 42 m/s for the US beam parallel to the artC surface , and 1574 + / - 29 , 1621 + / - 34 and 1701 + / - 36 m/s for the beam perpendicular to the artC surface .
	manualset3
228247	8	421274	7	NULL	NULL	0	NULL	1554 + / - 42 m/s	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The US speeds of artC from the superficial to deep regions were 1518 + / - 17 ( mean + SD ) , 1532 + / - 26 and 1554 + / - 42 m/s for the US beam parallel to the artC surface , and 1574 + / - 29 , 1621 + / - 34 and 1701 + / - 36 m/s for the beam perpendicular to the artC surface .
	manualset3
228248	9	421274	7	NULL	NULL	0	NULL	US beam	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The US speeds of artC from the superficial to deep regions were 1518 + / - 17 ( mean + SD ) , 1532 + / - 26 and 1554 + / - 42 m/s for the US beam parallel to the artC surface , and 1574 + / - 29 , 1621 + / - 34 and 1701 + / - 36 m/s for the beam perpendicular to the artC surface .
	manualset3
228249	10	421274	7	NULL	NULL	0	NULL	artC surface	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The US speeds of artC from the superficial to deep regions were 1518 + / - 17 ( mean + SD ) , 1532 + / - 26 and 1554 + / - 42 m/s for the US beam parallel to the artC surface , and 1574 + / - 29 , 1621 + / - 34 and 1701 + / - 36 m/s for the beam perpendicular to the artC surface .
	manualset3
228250	11	421274	7	NULL	NULL	0	NULL	1574 + / - 29 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The US speeds of artC from the superficial to deep regions were 1518 + / - 17 ( mean + SD ) , 1532 + / - 26 and 1554 + / - 42 m/s for the US beam parallel to the artC surface , and 1574 + / - 29 , 1621 + / - 34 and 1701 + / - 36 m/s for the beam perpendicular to the artC surface .
	manualset3
228251	12	421274	7	NULL	NULL	0	NULL	1621 + / - 34	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The US speeds of artC from the superficial to deep regions were 1518 + / - 17 ( mean + SD ) , 1532 + / - 26 and 1554 + / - 42 m/s for the US beam parallel to the artC surface , and 1574 + / - 29 , 1621 + / - 34 and 1701 + / - 36 m/s for the beam perpendicular to the artC surface .
	manualset3
228252	13	421274	7	NULL	NULL	0	NULL	1701 + / - 36 m/s	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The US speeds of artC from the superficial to deep regions were 1518 + / - 17 ( mean + SD ) , 1532 + / - 26 and 1554 + / - 42 m/s for the US beam parallel to the artC surface , and 1574 + / - 29 , 1621 + / - 34 and 1701 + / - 36 m/s for the beam perpendicular to the artC surface .
	manualset3
228253	14	421274	7	NULL	NULL	0	NULL	 beam	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The US speeds of artC from the superficial to deep regions were 1518 + / - 17 ( mean + SD ) , 1532 + / - 26 and 1554 + / - 42 m/s for the US beam parallel to the artC surface , and 1574 + / - 29 , 1621 + / - 34 and 1701 + / - 36 m/s for the beam perpendicular to the artC surface .
	manualset3
228254	15	421274	7	NULL	NULL	0	NULL	artC surface	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The US speeds of artC from the superficial to deep regions were 1518 + / - 17 ( mean + SD ) , 1532 + / - 26 and 1554 + / - 42 m/s for the US beam parallel to the artC surface , and 1574 + / - 29 , 1621 + / - 34 and 1701 + / - 36 m/s for the beam perpendicular to the artC surface .
	manualset3
228255	1	421275	7	NULL	NULL	0	NULL	selective mGluR5 agonist	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The selective mGluR5 agonist CHPG protects against traumatic brain injury in vitro and in vivo via ERK and Akt pathway .
	manualset3
228256	2	421275	7	NULL	NULL	0	NULL	CHPG	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The selective mGluR5 agonist CHPG protects against traumatic brain injury in vitro and in vivo via ERK and Akt pathway .
	manualset3
228257	3	421275	7	NULL	NULL	0	NULL	traumatic brain injury 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The selective mGluR5 agonist CHPG protects against traumatic brain injury in vitro and in vivo via ERK and Akt pathway .
	manualset3
228258	4	421275	7	NULL	NULL	0	NULL	ERK pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The selective mGluR5 agonist CHPG protects against traumatic brain injury in vitro and in vivo via ERK and Akt pathway .
	manualset3
228259	5	421275	7	NULL	NULL	0	NULL	Akt pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The selective mGluR5 agonist CHPG protects against traumatic brain injury in vitro and in vivo via ERK and Akt pathway .
	manualset3
228260	1	421276	7	NULL	NULL	0	NULL	high variability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although a high variability in the content of furosine was noticed , in general terms , the lowest levels of furosine were observed in samples of fruit-based infant foods and the highest were observed in jams of more than 60 % sugar .
	manualset3
228261	2	421276	7	NULL	NULL	0	NULL	 content 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although a high variability in the content of furosine was noticed , in general terms , the lowest levels of furosine were observed in samples of fruit-based infant foods and the highest were observed in jams of more than 60 % sugar .
	manualset3
228262	3	421276	7	NULL	NULL	0	NULL	furosine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although a high variability in the content of furosine was noticed , in general terms , the lowest levels of furosine were observed in samples of fruit-based infant foods and the highest were observed in jams of more than 60 % sugar .
	manualset3
228263	4	421276	7	NULL	NULL	0	NULL	general terms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although a high variability in the content of furosine was noticed , in general terms , the lowest levels of furosine were observed in samples of fruit-based infant foods and the highest were observed in jams of more than 60 % sugar .
	manualset3
228264	5	421276	7	NULL	NULL	0	NULL	lowest levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although a high variability in the content of furosine was noticed , in general terms , the lowest levels of furosine were observed in samples of fruit-based infant foods and the highest were observed in jams of more than 60 % sugar .
	manualset3
228265	6	421276	7	NULL	NULL	0	NULL	 furosine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although a high variability in the content of furosine was noticed , in general terms , the lowest levels of furosine were observed in samples of fruit-based infant foods and the highest were observed in jams of more than 60 % sugar .
	manualset3
228266	7	421276	7	NULL	NULL	0	NULL	samples	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Although a high variability in the content of furosine was noticed , in general terms , the lowest levels of furosine were observed in samples of fruit-based infant foods and the highest were observed in jams of more than 60 % sugar .
	manualset3
228267	8	421276	7	NULL	NULL	0	NULL	fruit-based infant foods	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Although a high variability in the content of furosine was noticed , in general terms , the lowest levels of furosine were observed in samples of fruit-based infant foods and the highest were observed in jams of more than 60 % sugar .
	manualset3
228268	9	421276	7	NULL	NULL	0	NULL	jams	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Although a high variability in the content of furosine was noticed , in general terms , the lowest levels of furosine were observed in samples of fruit-based infant foods and the highest were observed in jams of more than 60 % sugar .
	manualset3
228269	10	421276	7	NULL	NULL	0	NULL	60 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although a high variability in the content of furosine was noticed , in general terms , the lowest levels of furosine were observed in samples of fruit-based infant foods and the highest were observed in jams of more than 60 % sugar .
	manualset3
228270	11	421276	7	NULL	NULL	0	NULL	sugar	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Although a high variability in the content of furosine was noticed , in general terms , the lowest levels of furosine were observed in samples of fruit-based infant foods and the highest were observed in jams of more than 60 % sugar .
	manualset3
228271	1	421277	7	NULL	NULL	0	NULL	Clinical pharmacokinetics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical pharmacokinetics of meropenem and biapenem in bile and dosing considerations for biliary tract infections based on site-specific pharmacodynamic target attainment .
	manualset3
228272	2	421277	7	NULL	NULL	0	NULL	 meropenem	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical pharmacokinetics of meropenem and biapenem in bile and dosing considerations for biliary tract infections based on site-specific pharmacodynamic target attainment .
	manualset3
228273	3	421277	7	NULL	NULL	0	NULL	biapenem	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical pharmacokinetics of meropenem and biapenem in bile and dosing considerations for biliary tract infections based on site-specific pharmacodynamic target attainment .
	manualset3
228274	4	421277	7	NULL	NULL	0	NULL	bile	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical pharmacokinetics of meropenem and biapenem in bile and dosing considerations for biliary tract infections based on site-specific pharmacodynamic target attainment .
	manualset3
228275	5	421277	7	NULL	NULL	0	NULL	dosing considerations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical pharmacokinetics of meropenem and biapenem in bile and dosing considerations for biliary tract infections based on site-specific pharmacodynamic target attainment .
	manualset3
228276	6	421277	7	NULL	NULL	0	NULL	biliary tract infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical pharmacokinetics of meropenem and biapenem in bile and dosing considerations for biliary tract infections based on site-specific pharmacodynamic target attainment .
	manualset3
228277	7	421277	7	NULL	NULL	0	NULL	site-specific pharmacodynamic target attainment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical pharmacokinetics of meropenem and biapenem in bile and dosing considerations for biliary tract infections based on site-specific pharmacodynamic target attainment .
	manualset3
228278	1	421278	7	NULL	NULL	0	NULL	 generation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the generation of oxygenated radicals in dust-cell interactions has been demonstrated , there are no data correlating the toxicity of a dust with the level of oxygen radical generation by the dust during its interaction with phagocytic cells .
	manualset3
228279	2	421278	7	NULL	NULL	NULL	NULL	oxygenated radicals	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although the generation of oxygenated radicals in dust-cell interactions has been demonstrated , there are no data correlating the toxicity of a dust with the level of oxygen radical generation by the dust during its interaction with phagocytic cells .
	manualset3
228280	3	421278	7	NULL	NULL	0	NULL	dust-cell interactions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the generation of oxygenated radicals in dust-cell interactions has been demonstrated , there are no data correlating the toxicity of a dust with the level of oxygen radical generation by the dust during its interaction with phagocytic cells .
	manualset3
228281	4	421278	7	NULL	NULL	0	NULL	 no data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the generation of oxygenated radicals in dust-cell interactions has been demonstrated , there are no data correlating the toxicity of a dust with the level of oxygen radical generation by the dust during its interaction with phagocytic cells .
	manualset3
228282	5	421278	7	NULL	NULL	0	NULL	 toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the generation of oxygenated radicals in dust-cell interactions has been demonstrated , there are no data correlating the toxicity of a dust with the level of oxygen radical generation by the dust during its interaction with phagocytic cells .
	manualset3
228283	6	421278	7	NULL	NULL	0	NULL	dust	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the generation of oxygenated radicals in dust-cell interactions has been demonstrated , there are no data correlating the toxicity of a dust with the level of oxygen radical generation by the dust during its interaction with phagocytic cells .
	manualset3
228284	7	421278	7	NULL	NULL	0	NULL	level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the generation of oxygenated radicals in dust-cell interactions has been demonstrated , there are no data correlating the toxicity of a dust with the level of oxygen radical generation by the dust during its interaction with phagocytic cells .
	manualset3
228285	8	421278	7	NULL	NULL	0	NULL	oxygen radical generation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the generation of oxygenated radicals in dust-cell interactions has been demonstrated , there are no data correlating the toxicity of a dust with the level of oxygen radical generation by the dust during its interaction with phagocytic cells .
	manualset3
228286	9	421278	7	NULL	NULL	0	NULL	dust 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the generation of oxygenated radicals in dust-cell interactions has been demonstrated , there are no data correlating the toxicity of a dust with the level of oxygen radical generation by the dust during its interaction with phagocytic cells .
	manualset3
228287	10	421278	7	NULL	NULL	0	NULL	interaction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the generation of oxygenated radicals in dust-cell interactions has been demonstrated , there are no data correlating the toxicity of a dust with the level of oxygen radical generation by the dust during its interaction with phagocytic cells .
	manualset3
228288	11	421278	7	NULL	NULL	0	NULL	phagocytic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the generation of oxygenated radicals in dust-cell interactions has been demonstrated , there are no data correlating the toxicity of a dust with the level of oxygen radical generation by the dust during its interaction with phagocytic cells .
	manualset3
228289	1	421279	7	NULL	NULL	0	NULL	Heart rate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Heart rate increases by 4-8 beats per minute , on average , and the rate-pressure product and oxygen consumption increase by approximately 25 % .
	manualset3
228290	2	421279	7	NULL	NULL	0	NULL	4-8 beats per minute	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Heart rate increases by 4-8 beats per minute , on average , and the rate-pressure product and oxygen consumption increase by approximately 25 % .
	manualset3
228291	3	421279	7	NULL	NULL	0	NULL	average	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Heart rate increases by 4-8 beats per minute , on average , and the rate-pressure product and oxygen consumption increase by approximately 25 % .
	manualset3
228292	4	421279	7	NULL	NULL	0	NULL	 rate-pressure product	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Heart rate increases by 4-8 beats per minute , on average , and the rate-pressure product and oxygen consumption increase by approximately 25 % .
	manualset3
228293	5	421279	7	NULL	NULL	0	NULL	oxygen consumption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heart rate increases by 4-8 beats per minute , on average , and the rate-pressure product and oxygen consumption increase by approximately 25 % .
	manualset3
228294	6	421279	7	NULL	NULL	0	NULL	25 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Heart rate increases by 4-8 beats per minute , on average , and the rate-pressure product and oxygen consumption increase by approximately 25 % .
	manualset3
228295	1	421280	7	NULL	NULL	0	NULL	11-year-old girl	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	An 11-year-old girl presented with complaints of palpitations and cyanosis .
	manualset3
228296	2	421280	7	NULL	NULL	0	NULL	complaints	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An 11-year-old girl presented with complaints of palpitations and cyanosis .
	manualset3
228297	3	421280	7	NULL	NULL	0	NULL	palpitations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An 11-year-old girl presented with complaints of palpitations and cyanosis .
	manualset3
228298	4	421280	7	NULL	NULL	0	NULL	cyanosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An 11-year-old girl presented with complaints of palpitations and cyanosis .
	manualset3
228299	1	421281	7	NULL	NULL	0	NULL	Cholesterol synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cholesterol synthesis in brain , indicated by lathosterol , a local surrogate cholesterol synthesis marker , does not seem to be affected by plant sterol or stanol ester feeding .
	manualset3
228300	2	421281	7	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Cholesterol synthesis in brain , indicated by lathosterol , a local surrogate cholesterol synthesis marker , does not seem to be affected by plant sterol or stanol ester feeding .
	manualset3
228301	3	421281	7	NULL	NULL	0	NULL	 lathosterol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Cholesterol synthesis in brain , indicated by lathosterol , a local surrogate cholesterol synthesis marker , does not seem to be affected by plant sterol or stanol ester feeding .
	manualset3
228302	4	421281	7	NULL	NULL	0	NULL	local surrogate cholesterol synthesis marker	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Cholesterol synthesis in brain , indicated by lathosterol , a local surrogate cholesterol synthesis marker , does not seem to be affected by plant sterol or stanol ester feeding .
	manualset3
228303	5	421281	7	NULL	NULL	0	NULL	plant sterol 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Cholesterol synthesis in brain , indicated by lathosterol , a local surrogate cholesterol synthesis marker , does not seem to be affected by plant sterol or stanol ester feeding .
	manualset3
228304	6	421281	7	NULL	NULL	0	NULL	stanol ester feeding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cholesterol synthesis in brain , indicated by lathosterol , a local surrogate cholesterol synthesis marker , does not seem to be affected by plant sterol or stanol ester feeding .
	manualset3
228305	1	421282	7	NULL	NULL	0	NULL	Capacity factor	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Capacity factor was chosen as a dependent variable .
	manualset3
228306	2	421282	7	NULL	NULL	0	NULL	 dependent variable	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Capacity factor was chosen as a dependent variable .
	manualset3
228307	1	421283	7	NULL	NULL	0	NULL	ebselen	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , ebselen did not suppress plasma albumin extravasation into arthritic joints and dermal inflammatory reactions .
	manualset3
228308	2	421283	7	NULL	NULL	0	NULL	plasma albumin extravasation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , ebselen did not suppress plasma albumin extravasation into arthritic joints and dermal inflammatory reactions .
	manualset3
228309	3	421283	7	NULL	NULL	0	NULL	arthritic joints	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , ebselen did not suppress plasma albumin extravasation into arthritic joints and dermal inflammatory reactions .
	manualset3
228310	4	421283	7	NULL	NULL	0	NULL	dermal inflammatory reactions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , ebselen did not suppress plasma albumin extravasation into arthritic joints and dermal inflammatory reactions .
	manualset3
228311	1	421284	7	NULL	NULL	0	NULL	Preparation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Preparation of antibodies to catecholamines and metabolites -- syntheses of various immunogens and characterization of the resulting antibodies .
	manualset3
228312	2	421284	7	NULL	NULL	0	NULL	 antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Preparation of antibodies to catecholamines and metabolites -- syntheses of various immunogens and characterization of the resulting antibodies .
	manualset3
228313	3	421284	7	NULL	NULL	0	NULL	catecholamines	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Preparation of antibodies to catecholamines and metabolites -- syntheses of various immunogens and characterization of the resulting antibodies .
	manualset3
228314	4	421284	7	NULL	NULL	0	NULL	metabolites	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Preparation of antibodies to catecholamines and metabolites -- syntheses of various immunogens and characterization of the resulting antibodies .
	manualset3
228315	5	421284	7	NULL	NULL	0	NULL	syntheses	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Preparation of antibodies to catecholamines and metabolites -- syntheses of various immunogens and characterization of the resulting antibodies .
	manualset3
228316	6	421284	7	NULL	NULL	0	NULL	 immunogens 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Preparation of antibodies to catecholamines and metabolites -- syntheses of various immunogens and characterization of the resulting antibodies .
	manualset3
228317	7	421284	7	NULL	NULL	0	NULL	characterization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Preparation of antibodies to catecholamines and metabolites -- syntheses of various immunogens and characterization of the resulting antibodies .
	manualset3
228318	8	421284	7	NULL	NULL	0	NULL	antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Preparation of antibodies to catecholamines and metabolites -- syntheses of various immunogens and characterization of the resulting antibodies .
	manualset3
228319	1	421285	7	NULL	NULL	0	NULL	spatial Poisson point process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A spatial Poisson point process is employed to randomly locate vacancy defects on nanotubes .
	manualset3
228320	2	421285	7	NULL	NULL	0	NULL	 vacancy defects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A spatial Poisson point process is employed to randomly locate vacancy defects on nanotubes .
	manualset3
228321	3	421285	7	NULL	NULL	0	NULL	nanotubes	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A spatial Poisson point process is employed to randomly locate vacancy defects on nanotubes .
	manualset3
228322	1	421286	7	NULL	NULL	0	NULL	Serologic evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serologic evidence of Venezuelan equine encephalitis virus infections in raccoons of south central Florida .
	manualset3
228323	2	421286	7	NULL	NULL	0	NULL	Venezuelan equine encephalitis virus infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serologic evidence of Venezuelan equine encephalitis virus infections in raccoons of south central Florida .
	manualset3
228324	3	421286	7	NULL	NULL	0	NULL	raccoons	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Serologic evidence of Venezuelan equine encephalitis virus infections in raccoons of south central Florida .
	manualset3
228325	4	421286	7	NULL	NULL	0	NULL	south central Florida	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Serologic evidence of Venezuelan equine encephalitis virus infections in raccoons of south central Florida .
	manualset3
228326	1	421287	7	NULL	NULL	0	NULL	Histamine release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Histamine release by calcium from sodium fluoride-activated rat mast cells .
	manualset3
228327	2	421287	7	NULL	NULL	0	NULL	calcium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Histamine release by calcium from sodium fluoride-activated rat mast cells .
	manualset3
228328	3	421287	7	NULL	NULL	0	NULL	sodium fluoride-activated rat mast cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Histamine release by calcium from sodium fluoride-activated rat mast cells .
	manualset3
228329	1	421288	7	NULL	NULL	0	NULL	normal structure 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Despite an apparently normal structure , these spermatozoa had decreased motility and showed an increase in spontaneous acrosome reactions .
	manualset3
228330	2	421288	7	NULL	NULL	0	NULL	spermatozoa	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Despite an apparently normal structure , these spermatozoa had decreased motility and showed an increase in spontaneous acrosome reactions .
	manualset3
228331	3	421288	7	NULL	NULL	0	NULL	motility	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Despite an apparently normal structure , these spermatozoa had decreased motility and showed an increase in spontaneous acrosome reactions .
	manualset3
228332	4	421288	7	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Despite an apparently normal structure , these spermatozoa had decreased motility and showed an increase in spontaneous acrosome reactions .
	manualset3
228333	5	421288	7	NULL	NULL	0	NULL	spontaneous acrosome reactions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Despite an apparently normal structure , these spermatozoa had decreased motility and showed an increase in spontaneous acrosome reactions .
	manualset3
228334	1	421289	7	NULL	NULL	0	NULL	knockdown	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , knockdown or overexpression of the AKT downstream targets Foxo1 and Foxo3a was found to inhibit or promote iTreg differentiation in PKC - ( - / - ) T cells accordingly , indicating that the AKT-Foxo1 / 3A pathway is responsible for the inhibition of iTreg differentiation of iTregs downstream of PKC - .
	manualset3
228335	2	421289	7	NULL	NULL	0	NULL	overexpression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , knockdown or overexpression of the AKT downstream targets Foxo1 and Foxo3a was found to inhibit or promote iTreg differentiation in PKC - ( - / - ) T cells accordingly , indicating that the AKT-Foxo1 / 3A pathway is responsible for the inhibition of iTreg differentiation of iTregs downstream of PKC - .
	manualset3
228336	3	421289	7	NULL	NULL	0	NULL	AKT downstream targets	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , knockdown or overexpression of the AKT downstream targets Foxo1 and Foxo3a was found to inhibit or promote iTreg differentiation in PKC - ( - / - ) T cells accordingly , indicating that the AKT-Foxo1 / 3A pathway is responsible for the inhibition of iTreg differentiation of iTregs downstream of PKC - .
	manualset3
228337	4	421289	7	NULL	NULL	0	NULL	Foxo1	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , knockdown or overexpression of the AKT downstream targets Foxo1 and Foxo3a was found to inhibit or promote iTreg differentiation in PKC - ( - / - ) T cells accordingly , indicating that the AKT-Foxo1 / 3A pathway is responsible for the inhibition of iTreg differentiation of iTregs downstream of PKC - .
	manualset3
228338	5	421289	7	NULL	NULL	0	NULL	Foxo3a	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , knockdown or overexpression of the AKT downstream targets Foxo1 and Foxo3a was found to inhibit or promote iTreg differentiation in PKC - ( - / - ) T cells accordingly , indicating that the AKT-Foxo1 / 3A pathway is responsible for the inhibition of iTreg differentiation of iTregs downstream of PKC - .
	manualset3
228339	6	421289	7	NULL	NULL	0	NULL	iTreg differentiation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , knockdown or overexpression of the AKT downstream targets Foxo1 and Foxo3a was found to inhibit or promote iTreg differentiation in PKC - ( - / - ) T cells accordingly , indicating that the AKT-Foxo1 / 3A pathway is responsible for the inhibition of iTreg differentiation of iTregs downstream of PKC - .
	manualset3
228340	7	421289	7	NULL	NULL	0	NULL	PKC - ( - / - ) T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , knockdown or overexpression of the AKT downstream targets Foxo1 and Foxo3a was found to inhibit or promote iTreg differentiation in PKC - ( - / - ) T cells accordingly , indicating that the AKT-Foxo1 / 3A pathway is responsible for the inhibition of iTreg differentiation of iTregs downstream of PKC - .
	manualset3
228341	8	421289	7	NULL	NULL	0	NULL	AKT-Foxo1 / 3A pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , knockdown or overexpression of the AKT downstream targets Foxo1 and Foxo3a was found to inhibit or promote iTreg differentiation in PKC - ( - / - ) T cells accordingly , indicating that the AKT-Foxo1 / 3A pathway is responsible for the inhibition of iTreg differentiation of iTregs downstream of PKC - .
	manualset3
228342	9	421289	7	NULL	NULL	0	NULL	 inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , knockdown or overexpression of the AKT downstream targets Foxo1 and Foxo3a was found to inhibit or promote iTreg differentiation in PKC - ( - / - ) T cells accordingly , indicating that the AKT-Foxo1 / 3A pathway is responsible for the inhibition of iTreg differentiation of iTregs downstream of PKC - .
	manualset3
228343	10	421289	7	NULL	NULL	0	NULL	iTreg differentiation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , knockdown or overexpression of the AKT downstream targets Foxo1 and Foxo3a was found to inhibit or promote iTreg differentiation in PKC - ( - / - ) T cells accordingly , indicating that the AKT-Foxo1 / 3A pathway is responsible for the inhibition of iTreg differentiation of iTregs downstream of PKC - .
	manualset3
228344	11	421289	7	NULL	NULL	0	NULL	iTregs	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , knockdown or overexpression of the AKT downstream targets Foxo1 and Foxo3a was found to inhibit or promote iTreg differentiation in PKC - ( - / - ) T cells accordingly , indicating that the AKT-Foxo1 / 3A pathway is responsible for the inhibition of iTreg differentiation of iTregs downstream of PKC - .
	manualset3
228345	12	421289	7	NULL	NULL	0	NULL	PKC	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , knockdown or overexpression of the AKT downstream targets Foxo1 and Foxo3a was found to inhibit or promote iTreg differentiation in PKC - ( - / - ) T cells accordingly , indicating that the AKT-Foxo1 / 3A pathway is responsible for the inhibition of iTreg differentiation of iTregs downstream of PKC - .
	manualset3
228346	1	421290	7	NULL	NULL	0	NULL	Determination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of organochlorine pesticide residues in nine herbs by solid-phase extraction and capillary gas chromatography ) .
	manualset3
228347	2	421290	7	NULL	NULL	0	NULL	organochlorine pesticide residues	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of organochlorine pesticide residues in nine herbs by solid-phase extraction and capillary gas chromatography ) .
	manualset3
228348	3	421290	7	NULL	NULL	0	NULL	nine herbs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of organochlorine pesticide residues in nine herbs by solid-phase extraction and capillary gas chromatography ) .
	manualset3
228349	4	421290	7	NULL	NULL	0	NULL	solid-phase extraction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of organochlorine pesticide residues in nine herbs by solid-phase extraction and capillary gas chromatography ) .
	manualset3
228350	5	421290	7	NULL	NULL	0	NULL	capillary gas chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of organochlorine pesticide residues in nine herbs by solid-phase extraction and capillary gas chromatography ) .
	manualset3
228351	1	421291	7	NULL	NULL	0	NULL	 18-year-old female	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	An 18-year-old female and a 14-year-old male who had previously received surgery for primary repair of a nonsyndromic cleft lip and palate ( including alveolar defect bone grafting ) unintentionally developed facial advancement at the Le Fort III level after surgical correction of their maxillary hypoplasia .
	manualset3
228352	2	421291	7	NULL	NULL	0	NULL	14-year-old male	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	An 18-year-old female and a 14-year-old male who had previously received surgery for primary repair of a nonsyndromic cleft lip and palate ( including alveolar defect bone grafting ) unintentionally developed facial advancement at the Le Fort III level after surgical correction of their maxillary hypoplasia .
	manualset3
228353	3	421291	7	NULL	NULL	0	NULL	surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An 18-year-old female and a 14-year-old male who had previously received surgery for primary repair of a nonsyndromic cleft lip and palate ( including alveolar defect bone grafting ) unintentionally developed facial advancement at the Le Fort III level after surgical correction of their maxillary hypoplasia .
	manualset3
228354	4	421291	7	NULL	NULL	0	NULL	 primary repair	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An 18-year-old female and a 14-year-old male who had previously received surgery for primary repair of a nonsyndromic cleft lip and palate ( including alveolar defect bone grafting ) unintentionally developed facial advancement at the Le Fort III level after surgical correction of their maxillary hypoplasia .
	manualset3
228355	5	421291	7	NULL	NULL	0	NULL	nonsyndromic cleft lip 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An 18-year-old female and a 14-year-old male who had previously received surgery for primary repair of a nonsyndromic cleft lip and palate ( including alveolar defect bone grafting ) unintentionally developed facial advancement at the Le Fort III level after surgical correction of their maxillary hypoplasia .
	manualset3
228356	6	421291	7	NULL	NULL	0	NULL	 palate 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An 18-year-old female and a 14-year-old male who had previously received surgery for primary repair of a nonsyndromic cleft lip and palate ( including alveolar defect bone grafting ) unintentionally developed facial advancement at the Le Fort III level after surgical correction of their maxillary hypoplasia .
	manualset3
228357	7	421291	7	NULL	NULL	0	NULL	alveolar defect bone grafting	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An 18-year-old female and a 14-year-old male who had previously received surgery for primary repair of a nonsyndromic cleft lip and palate ( including alveolar defect bone grafting ) unintentionally developed facial advancement at the Le Fort III level after surgical correction of their maxillary hypoplasia .
	manualset3
228358	8	421291	7	NULL	NULL	NULL	NULL	facial advancement	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An 18-year-old female and a 14-year-old male who had previously received surgery for primary repair of a nonsyndromic cleft lip and palate ( including alveolar defect bone grafting ) unintentionally developed facial advancement at the Le Fort III level after surgical correction of their maxillary hypoplasia .
	manualset3
228359	9	421291	7	NULL	NULL	NULL	NULL	Le Fort III level	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An 18-year-old female and a 14-year-old male who had previously received surgery for primary repair of a nonsyndromic cleft lip and palate ( including alveolar defect bone grafting ) unintentionally developed facial advancement at the Le Fort III level after surgical correction of their maxillary hypoplasia .
	manualset3
228360	10	421291	7	NULL	NULL	0	NULL	 surgical correction	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An 18-year-old female and a 14-year-old male who had previously received surgery for primary repair of a nonsyndromic cleft lip and palate ( including alveolar defect bone grafting ) unintentionally developed facial advancement at the Le Fort III level after surgical correction of their maxillary hypoplasia .
	manualset3
228361	11	421291	7	NULL	NULL	0	NULL	maxillary hypoplasia .	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	An 18-year-old female and a 14-year-old male who had previously received surgery for primary repair of a nonsyndromic cleft lip and palate ( including alveolar defect bone grafting ) unintentionally developed facial advancement at the Le Fort III level after surgical correction of their maxillary hypoplasia .
	manualset3
228362	1	421292	7	NULL	NULL	0	NULL	Sixty-two patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty-two patients with advanced breast cancer were treated with either an endocrine ablative procedure or with antihormonal therapy .
	manualset3
228363	2	421292	7	NULL	NULL	0	NULL	advanced breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty-two patients with advanced breast cancer were treated with either an endocrine ablative procedure or with antihormonal therapy .
	manualset3
228364	3	421292	7	NULL	NULL	0	NULL	endocrine ablative procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty-two patients with advanced breast cancer were treated with either an endocrine ablative procedure or with antihormonal therapy .
	manualset3
228365	4	421292	7	NULL	NULL	0	NULL	antihormonal therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty-two patients with advanced breast cancer were treated with either an endocrine ablative procedure or with antihormonal therapy .
	manualset3
228366	1	421293	7	NULL	NULL	0	NULL	spontaneous plating efficiencies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We show here that based on the spontaneous plating efficiencies of their T-CFC , two groups of patients can be established : Group A ( 10 patients ) with a high colony number ( more than 100 colonies/10 ( 5 ) seeded cells ) , and group B ( 12 patients ) with less than 100 colonies/10 ( 5 ) cells .
	manualset3
228367	2	421293	7	NULL	NULL	0	NULL	T-CFC	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We show here that based on the spontaneous plating efficiencies of their T-CFC , two groups of patients can be established : Group A ( 10 patients ) with a high colony number ( more than 100 colonies/10 ( 5 ) seeded cells ) , and group B ( 12 patients ) with less than 100 colonies/10 ( 5 ) cells .
	manualset3
228368	3	421293	7	NULL	NULL	0	NULL	two groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We show here that based on the spontaneous plating efficiencies of their T-CFC , two groups of patients can be established : Group A ( 10 patients ) with a high colony number ( more than 100 colonies/10 ( 5 ) seeded cells ) , and group B ( 12 patients ) with less than 100 colonies/10 ( 5 ) cells .
	manualset3
228369	4	421293	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We show here that based on the spontaneous plating efficiencies of their T-CFC , two groups of patients can be established : Group A ( 10 patients ) with a high colony number ( more than 100 colonies/10 ( 5 ) seeded cells ) , and group B ( 12 patients ) with less than 100 colonies/10 ( 5 ) cells .
	manualset3
228370	5	421293	7	NULL	NULL	0	NULL	Group A	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We show here that based on the spontaneous plating efficiencies of their T-CFC , two groups of patients can be established : Group A ( 10 patients ) with a high colony number ( more than 100 colonies/10 ( 5 ) seeded cells ) , and group B ( 12 patients ) with less than 100 colonies/10 ( 5 ) cells .
	manualset3
228371	6	421293	7	NULL	NULL	0	NULL	10 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We show here that based on the spontaneous plating efficiencies of their T-CFC , two groups of patients can be established : Group A ( 10 patients ) with a high colony number ( more than 100 colonies/10 ( 5 ) seeded cells ) , and group B ( 12 patients ) with less than 100 colonies/10 ( 5 ) cells .
	manualset3
228372	7	421293	7	NULL	NULL	0	NULL	high colony number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We show here that based on the spontaneous plating efficiencies of their T-CFC , two groups of patients can be established : Group A ( 10 patients ) with a high colony number ( more than 100 colonies/10 ( 5 ) seeded cells ) , and group B ( 12 patients ) with less than 100 colonies/10 ( 5 ) cells .
	manualset3
228373	8	421293	7	NULL	NULL	0	NULL	100 colonies/10 ( 5 ) seeded cells 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We show here that based on the spontaneous plating efficiencies of their T-CFC , two groups of patients can be established : Group A ( 10 patients ) with a high colony number ( more than 100 colonies/10 ( 5 ) seeded cells ) , and group B ( 12 patients ) with less than 100 colonies/10 ( 5 ) cells .
	manualset3
228374	9	421293	7	NULL	NULL	0	NULL	group B	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We show here that based on the spontaneous plating efficiencies of their T-CFC , two groups of patients can be established : Group A ( 10 patients ) with a high colony number ( more than 100 colonies/10 ( 5 ) seeded cells ) , and group B ( 12 patients ) with less than 100 colonies/10 ( 5 ) cells .
	manualset3
228375	10	421293	7	NULL	NULL	0	NULL	12 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We show here that based on the spontaneous plating efficiencies of their T-CFC , two groups of patients can be established : Group A ( 10 patients ) with a high colony number ( more than 100 colonies/10 ( 5 ) seeded cells ) , and group B ( 12 patients ) with less than 100 colonies/10 ( 5 ) cells .
	manualset3
228376	11	421293	7	NULL	NULL	0	NULL	100 colonies/10 ( 5 ) cells 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We show here that based on the spontaneous plating efficiencies of their T-CFC , two groups of patients can be established : Group A ( 10 patients ) with a high colony number ( more than 100 colonies/10 ( 5 ) seeded cells ) , and group B ( 12 patients ) with less than 100 colonies/10 ( 5 ) cells .
	manualset3
228377	1	421294	7	NULL	NULL	0	NULL	complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Both were complications of ophthalmic surgical procedures that necessitated conjunctival incision .
	manualset3
228378	2	421294	7	NULL	NULL	0	NULL	 ophthalmic surgical procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Both were complications of ophthalmic surgical procedures that necessitated conjunctival incision .
	manualset3
228379	3	421294	7	NULL	NULL	0	NULL	conjunctival incision 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Both were complications of ophthalmic surgical procedures that necessitated conjunctival incision .
	manualset3
228380	1	421295	7	NULL	NULL	0	NULL	euchromatin	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	We found that the euchromatin in this X chromosome exhibited the same low sensitivity to DNase I as is characteristic of the inactive X chromosome .
	manualset3
228381	2	421295	7	NULL	NULL	0	NULL	X chromosome	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	We found that the euchromatin in this X chromosome exhibited the same low sensitivity to DNase I as is characteristic of the inactive X chromosome .
	manualset3
228382	3	421295	7	NULL	NULL	0	NULL	low sensitivity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We found that the euchromatin in this X chromosome exhibited the same low sensitivity to DNase I as is characteristic of the inactive X chromosome .
	manualset3
228383	4	421295	7	NULL	NULL	0	NULL	DNase I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We found that the euchromatin in this X chromosome exhibited the same low sensitivity to DNase I as is characteristic of the inactive X chromosome .
	manualset3
228384	5	421295	7	NULL	NULL	0	NULL	inactive X chromosome	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	We found that the euchromatin in this X chromosome exhibited the same low sensitivity to DNase I as is characteristic of the inactive X chromosome .
	manualset3
228385	1	421296	7	NULL	NULL	0	NULL	effectiveness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We examined an effectiveness of a new asthma telemedicine system in reducing hospitalizations using a multi-site randomized control study .
	manualset3
228386	2	421296	7	NULL	NULL	0	NULL	 new asthma telemedicine system 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	We examined an effectiveness of a new asthma telemedicine system in reducing hospitalizations using a multi-site randomized control study .
	manualset3
228387	3	421296	7	NULL	NULL	0	NULL	hospitalizations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We examined an effectiveness of a new asthma telemedicine system in reducing hospitalizations using a multi-site randomized control study .
	manualset3
228388	4	421296	7	NULL	NULL	0	NULL	multi-site randomized control study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We examined an effectiveness of a new asthma telemedicine system in reducing hospitalizations using a multi-site randomized control study .
	manualset3
228389	1	421297	7	NULL	NULL	0	NULL	Calcium-sensitive cytosolic phospholipase A2 ( cPLA2 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Calcium-sensitive cytosolic phospholipase A2 ( cPLA2 ) is responsible for receptor-mediated liberation of arachidonic acid , and thus plays an important role in the initiation of the inflammatory lipid-mediator cascade generating eicosanoids and platelet-activating factor .
	manualset3
228390	2	421297	7	NULL	NULL	0	NULL	receptor-mediated liberation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Calcium-sensitive cytosolic phospholipase A2 ( cPLA2 ) is responsible for receptor-mediated liberation of arachidonic acid , and thus plays an important role in the initiation of the inflammatory lipid-mediator cascade generating eicosanoids and platelet-activating factor .
	manualset3
228391	3	421297	7	NULL	NULL	0	NULL	arachidonic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Calcium-sensitive cytosolic phospholipase A2 ( cPLA2 ) is responsible for receptor-mediated liberation of arachidonic acid , and thus plays an important role in the initiation of the inflammatory lipid-mediator cascade generating eicosanoids and platelet-activating factor .
	manualset3
228392	4	421297	7	NULL	NULL	0	NULL	 important role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Calcium-sensitive cytosolic phospholipase A2 ( cPLA2 ) is responsible for receptor-mediated liberation of arachidonic acid , and thus plays an important role in the initiation of the inflammatory lipid-mediator cascade generating eicosanoids and platelet-activating factor .
	manualset3
228393	5	421297	7	NULL	NULL	0	NULL	initiation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Calcium-sensitive cytosolic phospholipase A2 ( cPLA2 ) is responsible for receptor-mediated liberation of arachidonic acid , and thus plays an important role in the initiation of the inflammatory lipid-mediator cascade generating eicosanoids and platelet-activating factor .
	manualset3
228394	6	421297	7	NULL	NULL	0	NULL	inflammatory lipid-mediator cascade	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Calcium-sensitive cytosolic phospholipase A2 ( cPLA2 ) is responsible for receptor-mediated liberation of arachidonic acid , and thus plays an important role in the initiation of the inflammatory lipid-mediator cascade generating eicosanoids and platelet-activating factor .
	manualset3
228395	7	421297	7	NULL	NULL	0	NULL	eicosanoids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Calcium-sensitive cytosolic phospholipase A2 ( cPLA2 ) is responsible for receptor-mediated liberation of arachidonic acid , and thus plays an important role in the initiation of the inflammatory lipid-mediator cascade generating eicosanoids and platelet-activating factor .
	manualset3
228396	8	421297	7	NULL	NULL	0	NULL	platelet-activating factor	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Calcium-sensitive cytosolic phospholipase A2 ( cPLA2 ) is responsible for receptor-mediated liberation of arachidonic acid , and thus plays an important role in the initiation of the inflammatory lipid-mediator cascade generating eicosanoids and platelet-activating factor .
	manualset3
228397	1	421298	7	NULL	NULL	0	NULL	Abnormal lymphocyte homing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Abnormal lymphocyte homing and colon lesions in ulcerative colitis : experiment with rats ) .
	manualset3
228398	2	421298	7	NULL	NULL	0	NULL	colon lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Abnormal lymphocyte homing and colon lesions in ulcerative colitis : experiment with rats ) .
	manualset3
228399	3	421298	7	NULL	NULL	0	NULL	ulcerative colitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Abnormal lymphocyte homing and colon lesions in ulcerative colitis : experiment with rats ) .
	manualset3
228400	4	421298	7	NULL	NULL	0	NULL	experiment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Abnormal lymphocyte homing and colon lesions in ulcerative colitis : experiment with rats ) .
	manualset3
228401	5	421298	7	NULL	NULL	0	NULL	rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Abnormal lymphocyte homing and colon lesions in ulcerative colitis : experiment with rats ) .
	manualset3
228402	1	421299	7	NULL	NULL	0	NULL	8-year-old boy	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	An 8-year-old boy presented with a 10-week history of ulcerating lesions which were histologically and immunocytochemically consistent with the diagnosis of angiocentric T-cell lymphoma .
	manualset3
228403	2	421299	7	NULL	NULL	0	NULL	10-week history	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An 8-year-old boy presented with a 10-week history of ulcerating lesions which were histologically and immunocytochemically consistent with the diagnosis of angiocentric T-cell lymphoma .
	manualset3
228404	3	421299	7	NULL	NULL	0	NULL	ulcerating lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An 8-year-old boy presented with a 10-week history of ulcerating lesions which were histologically and immunocytochemically consistent with the diagnosis of angiocentric T-cell lymphoma .
	manualset3
228405	4	421299	7	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An 8-year-old boy presented with a 10-week history of ulcerating lesions which were histologically and immunocytochemically consistent with the diagnosis of angiocentric T-cell lymphoma .
	manualset3
228406	5	421299	7	NULL	NULL	0	NULL	angiocentric T-cell lymphoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	An 8-year-old boy presented with a 10-week history of ulcerating lesions which were histologically and immunocytochemically consistent with the diagnosis of angiocentric T-cell lymphoma .
	manualset3
228407	1	421300	7	NULL	NULL	0	NULL	Multiple-dose administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple-dose administration of sitagliptin , a dipeptidyl peptidase-4 inhibitor , does not alter the single-dose pharmacokinetics of rosiglitazone in healthy subjects .
	manualset3
228408	2	421300	7	NULL	NULL	0	NULL	sitagliptin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple-dose administration of sitagliptin , a dipeptidyl peptidase-4 inhibitor , does not alter the single-dose pharmacokinetics of rosiglitazone in healthy subjects .
	manualset3
228409	3	421300	7	NULL	NULL	0	NULL	dipeptidyl peptidase-4 inhibitor	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple-dose administration of sitagliptin , a dipeptidyl peptidase-4 inhibitor , does not alter the single-dose pharmacokinetics of rosiglitazone in healthy subjects .
	manualset3
228410	4	421300	7	NULL	NULL	NULL	NULL	single-dose pharmacokinetics	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Multiple-dose administration of sitagliptin , a dipeptidyl peptidase-4 inhibitor , does not alter the single-dose pharmacokinetics of rosiglitazone in healthy subjects .
	manualset3
228411	5	421300	7	NULL	NULL	0	NULL	rosiglitazone 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple-dose administration of sitagliptin , a dipeptidyl peptidase-4 inhibitor , does not alter the single-dose pharmacokinetics of rosiglitazone in healthy subjects .
	manualset3
228412	6	421300	7	NULL	NULL	0	NULL	 healthy subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Multiple-dose administration of sitagliptin , a dipeptidyl peptidase-4 inhibitor , does not alter the single-dose pharmacokinetics of rosiglitazone in healthy subjects .
	manualset3
228413	1	421301	7	NULL	NULL	0	NULL	 effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of three doses ( 5 , 100 , and 250 micrograms/kg ) of pentagastrin on the activities of choline acetyltransferase ( ChAT ) and acetylcholine esterase ( AChE ) , the neurotransmitter enzymes that synthesize and degrade acetylcholine , and monoamine oxidase ( MAO ) , the degradation enzyme for catecholamines , were investigated .
	manualset3
228414	2	421301	7	NULL	NULL	0	NULL	three doses 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of three doses ( 5 , 100 , and 250 micrograms/kg ) of pentagastrin on the activities of choline acetyltransferase ( ChAT ) and acetylcholine esterase ( AChE ) , the neurotransmitter enzymes that synthesize and degrade acetylcholine , and monoamine oxidase ( MAO ) , the degradation enzyme for catecholamines , were investigated .
	manualset3
228415	3	421301	7	NULL	NULL	0	NULL	 5 micrograms/kg	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of three doses ( 5 , 100 , and 250 micrograms/kg ) of pentagastrin on the activities of choline acetyltransferase ( ChAT ) and acetylcholine esterase ( AChE ) , the neurotransmitter enzymes that synthesize and degrade acetylcholine , and monoamine oxidase ( MAO ) , the degradation enzyme for catecholamines , were investigated .
	manualset3
228416	4	421301	7	NULL	NULL	0	NULL	100 micrograms/kg	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of three doses ( 5 , 100 , and 250 micrograms/kg ) of pentagastrin on the activities of choline acetyltransferase ( ChAT ) and acetylcholine esterase ( AChE ) , the neurotransmitter enzymes that synthesize and degrade acetylcholine , and monoamine oxidase ( MAO ) , the degradation enzyme for catecholamines , were investigated .
	manualset3
228417	5	421301	7	NULL	NULL	0	NULL	250 micrograms/kg	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of three doses ( 5 , 100 , and 250 micrograms/kg ) of pentagastrin on the activities of choline acetyltransferase ( ChAT ) and acetylcholine esterase ( AChE ) , the neurotransmitter enzymes that synthesize and degrade acetylcholine , and monoamine oxidase ( MAO ) , the degradation enzyme for catecholamines , were investigated .
	manualset3
228418	6	421301	7	NULL	NULL	0	NULL	pentagastrin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of three doses ( 5 , 100 , and 250 micrograms/kg ) of pentagastrin on the activities of choline acetyltransferase ( ChAT ) and acetylcholine esterase ( AChE ) , the neurotransmitter enzymes that synthesize and degrade acetylcholine , and monoamine oxidase ( MAO ) , the degradation enzyme for catecholamines , were investigated .
	manualset3
228419	7	421301	7	NULL	NULL	0	NULL	activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of three doses ( 5 , 100 , and 250 micrograms/kg ) of pentagastrin on the activities of choline acetyltransferase ( ChAT ) and acetylcholine esterase ( AChE ) , the neurotransmitter enzymes that synthesize and degrade acetylcholine , and monoamine oxidase ( MAO ) , the degradation enzyme for catecholamines , were investigated .
	manualset3
228420	8	421301	7	NULL	NULL	0	NULL	choline acetyltransferase ( ChAT )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of three doses ( 5 , 100 , and 250 micrograms/kg ) of pentagastrin on the activities of choline acetyltransferase ( ChAT ) and acetylcholine esterase ( AChE ) , the neurotransmitter enzymes that synthesize and degrade acetylcholine , and monoamine oxidase ( MAO ) , the degradation enzyme for catecholamines , were investigated .
	manualset3
228421	9	421301	7	NULL	NULL	0	NULL	acetylcholine esterase ( AChE )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of three doses ( 5 , 100 , and 250 micrograms/kg ) of pentagastrin on the activities of choline acetyltransferase ( ChAT ) and acetylcholine esterase ( AChE ) , the neurotransmitter enzymes that synthesize and degrade acetylcholine , and monoamine oxidase ( MAO ) , the degradation enzyme for catecholamines , were investigated .
	manualset3
228422	10	421301	7	NULL	NULL	0	NULL	neurotransmitter enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of three doses ( 5 , 100 , and 250 micrograms/kg ) of pentagastrin on the activities of choline acetyltransferase ( ChAT ) and acetylcholine esterase ( AChE ) , the neurotransmitter enzymes that synthesize and degrade acetylcholine , and monoamine oxidase ( MAO ) , the degradation enzyme for catecholamines , were investigated .
	manualset3
228423	11	421301	7	NULL	NULL	0	NULL	acetylcholine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of three doses ( 5 , 100 , and 250 micrograms/kg ) of pentagastrin on the activities of choline acetyltransferase ( ChAT ) and acetylcholine esterase ( AChE ) , the neurotransmitter enzymes that synthesize and degrade acetylcholine , and monoamine oxidase ( MAO ) , the degradation enzyme for catecholamines , were investigated .
	manualset3
228424	12	421301	7	NULL	NULL	0	NULL	monoamine oxidase ( MAO )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of three doses ( 5 , 100 , and 250 micrograms/kg ) of pentagastrin on the activities of choline acetyltransferase ( ChAT ) and acetylcholine esterase ( AChE ) , the neurotransmitter enzymes that synthesize and degrade acetylcholine , and monoamine oxidase ( MAO ) , the degradation enzyme for catecholamines , were investigated .
	manualset3
228425	13	421301	7	NULL	NULL	0	NULL	degradation enzyme	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of three doses ( 5 , 100 , and 250 micrograms/kg ) of pentagastrin on the activities of choline acetyltransferase ( ChAT ) and acetylcholine esterase ( AChE ) , the neurotransmitter enzymes that synthesize and degrade acetylcholine , and monoamine oxidase ( MAO ) , the degradation enzyme for catecholamines , were investigated .
	manualset3
228426	14	421301	7	NULL	NULL	0	NULL	catecholamines	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of three doses ( 5 , 100 , and 250 micrograms/kg ) of pentagastrin on the activities of choline acetyltransferase ( ChAT ) and acetylcholine esterase ( AChE ) , the neurotransmitter enzymes that synthesize and degrade acetylcholine , and monoamine oxidase ( MAO ) , the degradation enzyme for catecholamines , were investigated .
	manualset3
228427	1	421302	7	NULL	NULL	0	NULL	vb relay cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to this , the vb relay cells were fired by ml impulses only once at short latencies , though later there occurred a series of two to three bursts of grouped discharges .
	manualset3
228428	2	421302	7	NULL	NULL	0	NULL	ml impulses	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to this , the vb relay cells were fired by ml impulses only once at short latencies , though later there occurred a series of two to three bursts of grouped discharges .
	manualset3
228429	3	421302	7	NULL	NULL	NULL	NULL	short latencies	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast to this , the vb relay cells were fired by ml impulses only once at short latencies , though later there occurred a series of two to three bursts of grouped discharges .
	manualset3
228430	4	421302	7	NULL	NULL	0	NULL	series	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to this , the vb relay cells were fired by ml impulses only once at short latencies , though later there occurred a series of two to three bursts of grouped discharges .
	manualset3
228431	5	421302	7	NULL	NULL	0	NULL	two bursts	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to this , the vb relay cells were fired by ml impulses only once at short latencies , though later there occurred a series of two to three bursts of grouped discharges .
	manualset3
228432	6	421302	7	NULL	NULL	0	NULL	three bursts 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to this , the vb relay cells were fired by ml impulses only once at short latencies , though later there occurred a series of two to three bursts of grouped discharges .
	manualset3
228433	7	421302	7	NULL	NULL	0	NULL	grouped discharges	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast to this , the vb relay cells were fired by ml impulses only once at short latencies , though later there occurred a series of two to three bursts of grouped discharges .
	manualset3
228434	1	421303	7	NULL	NULL	0	NULL	Serial electroencephalography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Serial electroencephalography in brain tumors and cerebrovascular accidents .
	manualset3
228435	2	421303	7	NULL	NULL	0	NULL	brain tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Serial electroencephalography in brain tumors and cerebrovascular accidents .
	manualset3
228436	3	421303	7	NULL	NULL	0	NULL	cerebrovascular accidents	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Serial electroencephalography in brain tumors and cerebrovascular accidents .
	manualset3
228437	1	421304	7	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of rolipram , a type IV phosphodiesterase inhibitor , on Pseudomonas aeruginosa infection of respiratory mucosa .
	manualset3
228438	2	421304	7	NULL	NULL	0	NULL	rolipram	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of rolipram , a type IV phosphodiesterase inhibitor , on Pseudomonas aeruginosa infection of respiratory mucosa .
	manualset3
228439	3	421304	7	NULL	NULL	0	NULL	type IV phosphodiesterase inhibitor	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of rolipram , a type IV phosphodiesterase inhibitor , on Pseudomonas aeruginosa infection of respiratory mucosa .
	manualset3
228440	4	421304	7	NULL	NULL	0	NULL	Pseudomonas aeruginosa infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of rolipram , a type IV phosphodiesterase inhibitor , on Pseudomonas aeruginosa infection of respiratory mucosa .
	manualset3
228441	5	421304	7	NULL	NULL	0	NULL	respiratory mucosa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of rolipram , a type IV phosphodiesterase inhibitor , on Pseudomonas aeruginosa infection of respiratory mucosa .
	manualset3
228442	1	421305	7	NULL	NULL	0	NULL	Hypothermia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothermia induced by THC ( 0.3 mg/kg , i.m. ) was prevented by Rimonabant ( 0.3 mg/kg , i.m. ) .
	manualset3
228443	2	421305	7	NULL	NULL	0	NULL	THC	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothermia induced by THC ( 0.3 mg/kg , i.m. ) was prevented by Rimonabant ( 0.3 mg/kg , i.m. ) .
	manualset3
228444	3	421305	7	NULL	NULL	0	NULL	0.3 mg/kg	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothermia induced by THC ( 0.3 mg/kg , i.m. ) was prevented by Rimonabant ( 0.3 mg/kg , i.m. ) .
	manualset3
228445	4	421305	7	NULL	NULL	0	NULL	i.m.	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothermia induced by THC ( 0.3 mg/kg , i.m. ) was prevented by Rimonabant ( 0.3 mg/kg , i.m. ) .
	manualset3
228446	5	421305	7	NULL	NULL	0	NULL	Rimonabant 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothermia induced by THC ( 0.3 mg/kg , i.m. ) was prevented by Rimonabant ( 0.3 mg/kg , i.m. ) .
	manualset3
228447	6	421305	7	NULL	NULL	0	NULL	0.3 mg/kg	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothermia induced by THC ( 0.3 mg/kg , i.m. ) was prevented by Rimonabant ( 0.3 mg/kg , i.m. ) .
	manualset3
228448	7	421305	7	NULL	NULL	0	NULL	i.m.	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypothermia induced by THC ( 0.3 mg/kg , i.m. ) was prevented by Rimonabant ( 0.3 mg/kg , i.m. ) .
	manualset3
228449	1	421306	7	NULL	NULL	0	NULL	four-fifths	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	About four-fifths of this funding came from State mental health agencies , with the remainder provided by sources such as State correctional agencies , State courts or other State sources , city/county jails , city/county courts , and other local public sources .
	manualset3
228450	2	421306	7	NULL	NULL	0	NULL	funding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	About four-fifths of this funding came from State mental health agencies , with the remainder provided by sources such as State correctional agencies , State courts or other State sources , city/county jails , city/county courts , and other local public sources .
	manualset3
228451	3	421306	7	NULL	NULL	0	NULL	State mental health agencies	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	About four-fifths of this funding came from State mental health agencies , with the remainder provided by sources such as State correctional agencies , State courts or other State sources , city/county jails , city/county courts , and other local public sources .
	manualset3
228452	4	421306	7	NULL	NULL	0	NULL	remainder	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	About four-fifths of this funding came from State mental health agencies , with the remainder provided by sources such as State correctional agencies , State courts or other State sources , city/county jails , city/county courts , and other local public sources .
	manualset3
228453	5	421306	7	NULL	NULL	0	NULL	sources	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	About four-fifths of this funding came from State mental health agencies , with the remainder provided by sources such as State correctional agencies , State courts or other State sources , city/county jails , city/county courts , and other local public sources .
	manualset3
228454	6	421306	7	NULL	NULL	0	NULL	State correctional agencies	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	About four-fifths of this funding came from State mental health agencies , with the remainder provided by sources such as State correctional agencies , State courts or other State sources , city/county jails , city/county courts , and other local public sources .
	manualset3
228455	7	421306	7	NULL	NULL	0	NULL	State courts	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	About four-fifths of this funding came from State mental health agencies , with the remainder provided by sources such as State correctional agencies , State courts or other State sources , city/county jails , city/county courts , and other local public sources .
	manualset3
228456	8	421306	7	NULL	NULL	0	NULL	State sources	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	About four-fifths of this funding came from State mental health agencies , with the remainder provided by sources such as State correctional agencies , State courts or other State sources , city/county jails , city/county courts , and other local public sources .
	manualset3
228457	9	421306	7	NULL	NULL	0	NULL	city/county jails	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	About four-fifths of this funding came from State mental health agencies , with the remainder provided by sources such as State correctional agencies , State courts or other State sources , city/county jails , city/county courts , and other local public sources .
	manualset3
228458	10	421306	7	NULL	NULL	0	NULL	 city/county courts	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	About four-fifths of this funding came from State mental health agencies , with the remainder provided by sources such as State correctional agencies , State courts or other State sources , city/county jails , city/county courts , and other local public sources .
	manualset3
228459	11	421306	7	NULL	NULL	0	NULL	local public sources	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	About four-fifths of this funding came from State mental health agencies , with the remainder provided by sources such as State correctional agencies , State courts or other State sources , city/county jails , city/county courts , and other local public sources .
	manualset3
228460	1	421307	7	NULL	NULL	0	NULL	 14	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the remaining 14 , six were found positive for C. trachomatis and were excluded as they did not return for the follow-up visit , one patient did not achieve complete eradication , one patient infected with both C. trachomatis and U. urealyticum failed to achieve complete eradication , and six patients infected with U. urealyticum failed to be completely cured .
	manualset3
228461	2	421307	7	NULL	NULL	0	NULL	six	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the remaining 14 , six were found positive for C. trachomatis and were excluded as they did not return for the follow-up visit , one patient did not achieve complete eradication , one patient infected with both C. trachomatis and U. urealyticum failed to achieve complete eradication , and six patients infected with U. urealyticum failed to be completely cured .
	manualset3
228462	3	421307	7	NULL	NULL	0	NULL	positive	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the remaining 14 , six were found positive for C. trachomatis and were excluded as they did not return for the follow-up visit , one patient did not achieve complete eradication , one patient infected with both C. trachomatis and U. urealyticum failed to achieve complete eradication , and six patients infected with U. urealyticum failed to be completely cured .
	manualset3
228463	4	421307	7	NULL	NULL	0	NULL	C. trachomatis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the remaining 14 , six were found positive for C. trachomatis and were excluded as they did not return for the follow-up visit , one patient did not achieve complete eradication , one patient infected with both C. trachomatis and U. urealyticum failed to achieve complete eradication , and six patients infected with U. urealyticum failed to be completely cured .
	manualset3
228464	5	421307	7	NULL	NULL	0	NULL	follow-up visit	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the remaining 14 , six were found positive for C. trachomatis and were excluded as they did not return for the follow-up visit , one patient did not achieve complete eradication , one patient infected with both C. trachomatis and U. urealyticum failed to achieve complete eradication , and six patients infected with U. urealyticum failed to be completely cured .
	manualset3
228465	6	421307	7	NULL	NULL	0	NULL	one patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the remaining 14 , six were found positive for C. trachomatis and were excluded as they did not return for the follow-up visit , one patient did not achieve complete eradication , one patient infected with both C. trachomatis and U. urealyticum failed to achieve complete eradication , and six patients infected with U. urealyticum failed to be completely cured .
	manualset3
228466	7	421307	7	NULL	NULL	0	NULL	complete eradication	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the remaining 14 , six were found positive for C. trachomatis and were excluded as they did not return for the follow-up visit , one patient did not achieve complete eradication , one patient infected with both C. trachomatis and U. urealyticum failed to achieve complete eradication , and six patients infected with U. urealyticum failed to be completely cured .
	manualset3
228467	8	421307	7	NULL	NULL	0	NULL	one patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the remaining 14 , six were found positive for C. trachomatis and were excluded as they did not return for the follow-up visit , one patient did not achieve complete eradication , one patient infected with both C. trachomatis and U. urealyticum failed to achieve complete eradication , and six patients infected with U. urealyticum failed to be completely cured .
	manualset3
228468	9	421307	7	NULL	NULL	0	NULL	C. trachomatis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the remaining 14 , six were found positive for C. trachomatis and were excluded as they did not return for the follow-up visit , one patient did not achieve complete eradication , one patient infected with both C. trachomatis and U. urealyticum failed to achieve complete eradication , and six patients infected with U. urealyticum failed to be completely cured .
	manualset3
228469	10	421307	7	NULL	NULL	0	NULL	U. urealyticum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the remaining 14 , six were found positive for C. trachomatis and were excluded as they did not return for the follow-up visit , one patient did not achieve complete eradication , one patient infected with both C. trachomatis and U. urealyticum failed to achieve complete eradication , and six patients infected with U. urealyticum failed to be completely cured .
	manualset3
228470	11	421307	7	NULL	NULL	0	NULL	complete eradication	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the remaining 14 , six were found positive for C. trachomatis and were excluded as they did not return for the follow-up visit , one patient did not achieve complete eradication , one patient infected with both C. trachomatis and U. urealyticum failed to achieve complete eradication , and six patients infected with U. urealyticum failed to be completely cured .
	manualset3
228471	12	421307	7	NULL	NULL	0	NULL	six patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the remaining 14 , six were found positive for C. trachomatis and were excluded as they did not return for the follow-up visit , one patient did not achieve complete eradication , one patient infected with both C. trachomatis and U. urealyticum failed to achieve complete eradication , and six patients infected with U. urealyticum failed to be completely cured .
	manualset3
228472	13	421307	7	NULL	NULL	0	NULL	U. urealyticum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the remaining 14 , six were found positive for C. trachomatis and were excluded as they did not return for the follow-up visit , one patient did not achieve complete eradication , one patient infected with both C. trachomatis and U. urealyticum failed to achieve complete eradication , and six patients infected with U. urealyticum failed to be completely cured .
	manualset3
228473	1	421308	7	NULL	NULL	0	NULL	key property 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A key property possessed by the mammalian cochlea is its ability to dynamically alter its own sensitivity .
	manualset3
228474	2	421308	7	NULL	NULL	0	NULL	mammalian cochlea	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A key property possessed by the mammalian cochlea is its ability to dynamically alter its own sensitivity .
	manualset3
228475	3	421308	7	NULL	NULL	0	NULL	 ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A key property possessed by the mammalian cochlea is its ability to dynamically alter its own sensitivity .
	manualset3
228476	4	421308	7	NULL	NULL	0	NULL	sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A key property possessed by the mammalian cochlea is its ability to dynamically alter its own sensitivity .
	manualset3
228477	1	421309	7	NULL	NULL	0	NULL	 method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , a method was developed , first , to obtain the power in the EEG frequency bands by digital filtering and , second , to display band-indices and ratios during a dive , in a format suitable for rapid appraisal .
	manualset3
228478	2	421309	7	NULL	NULL	0	NULL	power 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , a method was developed , first , to obtain the power in the EEG frequency bands by digital filtering and , second , to display band-indices and ratios during a dive , in a format suitable for rapid appraisal .
	manualset3
228479	3	421309	7	NULL	NULL	0	NULL	 EEG frequency bands	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , a method was developed , first , to obtain the power in the EEG frequency bands by digital filtering and , second , to display band-indices and ratios during a dive , in a format suitable for rapid appraisal .
	manualset3
228480	4	421309	7	NULL	NULL	0	NULL	digital filtering 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , a method was developed , first , to obtain the power in the EEG frequency bands by digital filtering and , second , to display band-indices and ratios during a dive , in a format suitable for rapid appraisal .
	manualset3
228481	5	421309	7	NULL	NULL	0	NULL	band-indices	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , a method was developed , first , to obtain the power in the EEG frequency bands by digital filtering and , second , to display band-indices and ratios during a dive , in a format suitable for rapid appraisal .
	manualset3
228482	6	421309	7	NULL	NULL	0	NULL	 ratios	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , a method was developed , first , to obtain the power in the EEG frequency bands by digital filtering and , second , to display band-indices and ratios during a dive , in a format suitable for rapid appraisal .
	manualset3
228483	7	421309	7	NULL	NULL	0	NULL	dive	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , a method was developed , first , to obtain the power in the EEG frequency bands by digital filtering and , second , to display band-indices and ratios during a dive , in a format suitable for rapid appraisal .
	manualset3
228484	9	421309	7	NULL	NULL	NULL	NULL	rapid appraisal	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Therefore , a method was developed , first , to obtain the power in the EEG frequency bands by digital filtering and , second , to display band-indices and ratios during a dive , in a format suitable for rapid appraisal .
	manualset3
228485	8	421309	7	NULL	NULL	0	NULL	format	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , a method was developed , first , to obtain the power in the EEG frequency bands by digital filtering and , second , to display band-indices and ratios during a dive , in a format suitable for rapid appraisal .
	manualset3
228486	1	421310	7	NULL	NULL	0	NULL	Congenital absence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Congenital absence of tibia is a rare anomaly .
	manualset3
228487	2	421310	7	NULL	NULL	0	NULL	tibia	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Congenital absence of tibia is a rare anomaly .
	manualset3
228488	3	421310	7	NULL	NULL	NULL	NULL	 rare anomaly	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Congenital absence of tibia is a rare anomaly .
	manualset3
228489	1	421311	7	NULL	NULL	0	NULL	44 kd species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The 44 kd species is distinct from the major intracellular forms of int-1 protein as judged by its slower mobility in SDS-polyacrylamide gels and by its longer half-life in pulse-chase experiments .
	manualset3
228490	2	421311	7	NULL	NULL	0	NULL	major intracellular forms 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The 44 kd species is distinct from the major intracellular forms of int-1 protein as judged by its slower mobility in SDS-polyacrylamide gels and by its longer half-life in pulse-chase experiments .
	manualset3
228491	3	421311	7	NULL	NULL	0	NULL	int-1 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The 44 kd species is distinct from the major intracellular forms of int-1 protein as judged by its slower mobility in SDS-polyacrylamide gels and by its longer half-life in pulse-chase experiments .
	manualset3
228492	4	421311	7	NULL	NULL	0	NULL	 slower mobility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 44 kd species is distinct from the major intracellular forms of int-1 protein as judged by its slower mobility in SDS-polyacrylamide gels and by its longer half-life in pulse-chase experiments .
	manualset3
228493	5	421311	7	NULL	NULL	0	NULL	SDS-polyacrylamide gels	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The 44 kd species is distinct from the major intracellular forms of int-1 protein as judged by its slower mobility in SDS-polyacrylamide gels and by its longer half-life in pulse-chase experiments .
	manualset3
228494	6	421311	7	NULL	NULL	0	NULL	longer half-life 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The 44 kd species is distinct from the major intracellular forms of int-1 protein as judged by its slower mobility in SDS-polyacrylamide gels and by its longer half-life in pulse-chase experiments .
	manualset3
228495	7	421311	7	NULL	NULL	0	NULL	pulse-chase experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The 44 kd species is distinct from the major intracellular forms of int-1 protein as judged by its slower mobility in SDS-polyacrylamide gels and by its longer half-life in pulse-chase experiments .
	manualset3
228496	1	421312	7	NULL	NULL	0	NULL	A * protein-ssDNA complex	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	An A * protein-ssDNA complex was isolated by gel filtration and shown to be active in a ligating reaction in which the two ends of the DNA fragment were joined to form a covalently closed circle .
	manualset3
228497	2	421312	7	NULL	NULL	0	NULL	gel filtration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An A * protein-ssDNA complex was isolated by gel filtration and shown to be active in a ligating reaction in which the two ends of the DNA fragment were joined to form a covalently closed circle .
	manualset3
228498	3	421312	7	NULL	NULL	0	NULL	ligating reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An A * protein-ssDNA complex was isolated by gel filtration and shown to be active in a ligating reaction in which the two ends of the DNA fragment were joined to form a covalently closed circle .
	manualset3
228499	4	421312	7	NULL	NULL	0	NULL	two ends	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	An A * protein-ssDNA complex was isolated by gel filtration and shown to be active in a ligating reaction in which the two ends of the DNA fragment were joined to form a covalently closed circle .
	manualset3
228500	5	421312	7	NULL	NULL	0	NULL	DNA fragment	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	An A * protein-ssDNA complex was isolated by gel filtration and shown to be active in a ligating reaction in which the two ends of the DNA fragment were joined to form a covalently closed circle .
	manualset3
228501	6	421312	7	NULL	NULL	0	NULL	covalently closed circle 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	An A * protein-ssDNA complex was isolated by gel filtration and shown to be active in a ligating reaction in which the two ends of the DNA fragment were joined to form a covalently closed circle .
	manualset3
228502	1	421313	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that SK channels are much more sensitive to Cd2 + than BK channels and indicate that Cd2 + is a selective agonist of SK channels .
	manualset3
228503	2	421313	7	NULL	NULL	0	NULL	SK channels 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that SK channels are much more sensitive to Cd2 + than BK channels and indicate that Cd2 + is a selective agonist of SK channels .
	manualset3
228504	3	421313	7	NULL	NULL	0	NULL	Cd2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that SK channels are much more sensitive to Cd2 + than BK channels and indicate that Cd2 + is a selective agonist of SK channels .
	manualset3
228505	4	421313	7	NULL	NULL	0	NULL	BK channels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that SK channels are much more sensitive to Cd2 + than BK channels and indicate that Cd2 + is a selective agonist of SK channels .
	manualset3
228506	5	421313	7	NULL	NULL	0	NULL	Cd2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that SK channels are much more sensitive to Cd2 + than BK channels and indicate that Cd2 + is a selective agonist of SK channels .
	manualset3
228507	6	421313	7	NULL	NULL	0	NULL	selective agonist	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that SK channels are much more sensitive to Cd2 + than BK channels and indicate that Cd2 + is a selective agonist of SK channels .
	manualset3
228508	7	421313	7	NULL	NULL	0	NULL	SK channels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The results show that SK channels are much more sensitive to Cd2 + than BK channels and indicate that Cd2 + is a selective agonist of SK channels .
	manualset3
228509	1	421314	7	NULL	NULL	0	NULL	swimming	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The swimming started 1 hour or 3 days after injury .
	manualset3
228510	2	421314	7	NULL	NULL	0	NULL	1 hour 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The swimming started 1 hour or 3 days after injury .
	manualset3
228511	3	421314	7	NULL	NULL	0	NULL	 3 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The swimming started 1 hour or 3 days after injury .
	manualset3
228512	4	421314	7	NULL	NULL	0	NULL	injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The swimming started 1 hour or 3 days after injury .
	manualset3
228513	1	421315	7	NULL	NULL	0	NULL	child	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Each child performed the modified Clinical Test of Sensory Interaction on Balance ( mCTSIB ) , Unilateral Stance ( US ) and Tandem Stance on ACG , mCTSIB and US on BBM and clinical balance tests : one-leg standing , balance beam walking and one-leg hopping .
	manualset3
228514	2	421315	7	NULL	NULL	0	NULL	modified Clinical Test of Sensory Interaction on Balance ( mCTSIB )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Each child performed the modified Clinical Test of Sensory Interaction on Balance ( mCTSIB ) , Unilateral Stance ( US ) and Tandem Stance on ACG , mCTSIB and US on BBM and clinical balance tests : one-leg standing , balance beam walking and one-leg hopping .
	manualset3
228515	3	421315	7	NULL	NULL	0	NULL	Unilateral Stance ( US ) 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Each child performed the modified Clinical Test of Sensory Interaction on Balance ( mCTSIB ) , Unilateral Stance ( US ) and Tandem Stance on ACG , mCTSIB and US on BBM and clinical balance tests : one-leg standing , balance beam walking and one-leg hopping .
	manualset3
228516	4	421315	7	NULL	NULL	0	NULL	Tandem Stance	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Each child performed the modified Clinical Test of Sensory Interaction on Balance ( mCTSIB ) , Unilateral Stance ( US ) and Tandem Stance on ACG , mCTSIB and US on BBM and clinical balance tests : one-leg standing , balance beam walking and one-leg hopping .
	manualset3
228517	5	421315	7	NULL	NULL	0	NULL	ACG	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Each child performed the modified Clinical Test of Sensory Interaction on Balance ( mCTSIB ) , Unilateral Stance ( US ) and Tandem Stance on ACG , mCTSIB and US on BBM and clinical balance tests : one-leg standing , balance beam walking and one-leg hopping .
	manualset3
228518	6	421315	7	NULL	NULL	0	NULL	mCTSIB 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Each child performed the modified Clinical Test of Sensory Interaction on Balance ( mCTSIB ) , Unilateral Stance ( US ) and Tandem Stance on ACG , mCTSIB and US on BBM and clinical balance tests : one-leg standing , balance beam walking and one-leg hopping .
	manualset3
228519	7	421315	7	NULL	NULL	0	NULL	US	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Each child performed the modified Clinical Test of Sensory Interaction on Balance ( mCTSIB ) , Unilateral Stance ( US ) and Tandem Stance on ACG , mCTSIB and US on BBM and clinical balance tests : one-leg standing , balance beam walking and one-leg hopping .
	manualset3
228520	8	421315	7	NULL	NULL	0	NULL	BBM	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Each child performed the modified Clinical Test of Sensory Interaction on Balance ( mCTSIB ) , Unilateral Stance ( US ) and Tandem Stance on ACG , mCTSIB and US on BBM and clinical balance tests : one-leg standing , balance beam walking and one-leg hopping .
	manualset3
228521	9	421315	7	NULL	NULL	0	NULL	clinical balance tests	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Each child performed the modified Clinical Test of Sensory Interaction on Balance ( mCTSIB ) , Unilateral Stance ( US ) and Tandem Stance on ACG , mCTSIB and US on BBM and clinical balance tests : one-leg standing , balance beam walking and one-leg hopping .
	manualset3
228522	10	421315	7	NULL	NULL	0	NULL	one-leg standing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Each child performed the modified Clinical Test of Sensory Interaction on Balance ( mCTSIB ) , Unilateral Stance ( US ) and Tandem Stance on ACG , mCTSIB and US on BBM and clinical balance tests : one-leg standing , balance beam walking and one-leg hopping .
	manualset3
228523	11	421315	7	NULL	NULL	0	NULL	balance beam walking	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Each child performed the modified Clinical Test of Sensory Interaction on Balance ( mCTSIB ) , Unilateral Stance ( US ) and Tandem Stance on ACG , mCTSIB and US on BBM and clinical balance tests : one-leg standing , balance beam walking and one-leg hopping .
	manualset3
228524	12	421315	7	NULL	NULL	0	NULL	one-leg hopping	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Each child performed the modified Clinical Test of Sensory Interaction on Balance ( mCTSIB ) , Unilateral Stance ( US ) and Tandem Stance on ACG , mCTSIB and US on BBM and clinical balance tests : one-leg standing , balance beam walking and one-leg hopping .
	manualset3
228525	1	421316	7	NULL	NULL	0	NULL	MR cholangiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	MR cholangiography in the evaluation of hepatic and biliary abnormalities in autosomal dominant polycystic kidney disease : study of 93 patients .
	manualset3
228526	2	421316	7	NULL	NULL	0	NULL	evaluation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	MR cholangiography in the evaluation of hepatic and biliary abnormalities in autosomal dominant polycystic kidney disease : study of 93 patients .
	manualset3
228527	3	421316	7	NULL	NULL	0	NULL	hepatic abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MR cholangiography in the evaluation of hepatic and biliary abnormalities in autosomal dominant polycystic kidney disease : study of 93 patients .
	manualset3
228528	4	421316	7	NULL	NULL	0	NULL	biliary abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	MR cholangiography in the evaluation of hepatic and biliary abnormalities in autosomal dominant polycystic kidney disease : study of 93 patients .
	manualset3
228529	5	421316	7	NULL	NULL	0	NULL	autosomal dominant polycystic kidney disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	MR cholangiography in the evaluation of hepatic and biliary abnormalities in autosomal dominant polycystic kidney disease : study of 93 patients .
	manualset3
228530	6	421316	7	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	MR cholangiography in the evaluation of hepatic and biliary abnormalities in autosomal dominant polycystic kidney disease : study of 93 patients .
	manualset3
228531	7	421316	7	NULL	NULL	0	NULL	93 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	MR cholangiography in the evaluation of hepatic and biliary abnormalities in autosomal dominant polycystic kidney disease : study of 93 patients .
	manualset3
228532	1	421317	7	NULL	NULL	0	NULL	Diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Diagnosis of hyper transaminasemia in childhood ) .
	manualset3
228533	2	421317	7	NULL	NULL	0	NULL	hyper transaminasemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Diagnosis of hyper transaminasemia in childhood ) .
	manualset3
228534	3	421317	7	NULL	NULL	0	NULL	childhood 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	( Diagnosis of hyper transaminasemia in childhood ) .
	manualset3
228535	1	421318	7	NULL	NULL	0	NULL	Potential microbial routes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential microbial routes to the production of plastics and synthetic fibers can be divided into three categories .
	manualset3
228536	2	421318	7	NULL	NULL	0	NULL	production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential microbial routes to the production of plastics and synthetic fibers can be divided into three categories .
	manualset3
228537	3	421318	7	NULL	NULL	0	NULL	plastics	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential microbial routes to the production of plastics and synthetic fibers can be divided into three categories .
	manualset3
228538	4	421318	7	NULL	NULL	0	NULL	synthetic fibers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential microbial routes to the production of plastics and synthetic fibers can be divided into three categories .
	manualset3
228539	5	421318	7	NULL	NULL	0	NULL	three categories	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Potential microbial routes to the production of plastics and synthetic fibers can be divided into three categories .
	manualset3
228540	1	421319	7	NULL	NULL	0	NULL	latrunculin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon removing latrunculin , hyperbranching produced abundant polar branches with normal F-actin organization throughout the colony .
	manualset3
228541	2	421319	7	NULL	NULL	NULL	NULL	hyperbranching	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Upon removing latrunculin , hyperbranching produced abundant polar branches with normal F-actin organization throughout the colony .
	manualset3
228542	3	421319	7	NULL	NULL	NULL	NULL	 polar branches	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Upon removing latrunculin , hyperbranching produced abundant polar branches with normal F-actin organization throughout the colony .
	manualset3
228543	4	421319	7	NULL	NULL	0	NULL	normal F-actin organization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon removing latrunculin , hyperbranching produced abundant polar branches with normal F-actin organization throughout the colony .
	manualset3
228544	5	421319	7	NULL	NULL	0	NULL	colony	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Upon removing latrunculin , hyperbranching produced abundant polar branches with normal F-actin organization throughout the colony .
	manualset3
228545	1	421320	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the lipophilicity and steric bulk of the terminal ring system , the amount of pi-electron density in the terminal ring , and the relative spatial proximity of the tetrazolyl and the middle phenyl are explored in terms of binding affinity to AT1 receptors in rat adrenal glomerulosa and rabbit aorta .
	manualset3
228546	2	421320	7	NULL	NULL	0	NULL	lipophilicity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the lipophilicity and steric bulk of the terminal ring system , the amount of pi-electron density in the terminal ring , and the relative spatial proximity of the tetrazolyl and the middle phenyl are explored in terms of binding affinity to AT1 receptors in rat adrenal glomerulosa and rabbit aorta .
	manualset3
228547	3	421320	7	NULL	NULL	0	NULL	steric bulk	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the lipophilicity and steric bulk of the terminal ring system , the amount of pi-electron density in the terminal ring , and the relative spatial proximity of the tetrazolyl and the middle phenyl are explored in terms of binding affinity to AT1 receptors in rat adrenal glomerulosa and rabbit aorta .
	manualset3
228548	4	421320	7	NULL	NULL	0	NULL	 terminal ring system	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the lipophilicity and steric bulk of the terminal ring system , the amount of pi-electron density in the terminal ring , and the relative spatial proximity of the tetrazolyl and the middle phenyl are explored in terms of binding affinity to AT1 receptors in rat adrenal glomerulosa and rabbit aorta .
	manualset3
228549	5	421320	7	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the lipophilicity and steric bulk of the terminal ring system , the amount of pi-electron density in the terminal ring , and the relative spatial proximity of the tetrazolyl and the middle phenyl are explored in terms of binding affinity to AT1 receptors in rat adrenal glomerulosa and rabbit aorta .
	manualset3
228550	6	421320	7	NULL	NULL	0	NULL	pi-electron density	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the lipophilicity and steric bulk of the terminal ring system , the amount of pi-electron density in the terminal ring , and the relative spatial proximity of the tetrazolyl and the middle phenyl are explored in terms of binding affinity to AT1 receptors in rat adrenal glomerulosa and rabbit aorta .
	manualset3
228551	7	421320	7	NULL	NULL	0	NULL	terminal ring	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the lipophilicity and steric bulk of the terminal ring system , the amount of pi-electron density in the terminal ring , and the relative spatial proximity of the tetrazolyl and the middle phenyl are explored in terms of binding affinity to AT1 receptors in rat adrenal glomerulosa and rabbit aorta .
	manualset3
228552	8	421320	7	NULL	NULL	0	NULL	 relative spatial proximity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the lipophilicity and steric bulk of the terminal ring system , the amount of pi-electron density in the terminal ring , and the relative spatial proximity of the tetrazolyl and the middle phenyl are explored in terms of binding affinity to AT1 receptors in rat adrenal glomerulosa and rabbit aorta .
	manualset3
228553	9	421320	7	NULL	NULL	0	NULL	tetrazolyl 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the lipophilicity and steric bulk of the terminal ring system , the amount of pi-electron density in the terminal ring , and the relative spatial proximity of the tetrazolyl and the middle phenyl are explored in terms of binding affinity to AT1 receptors in rat adrenal glomerulosa and rabbit aorta .
	manualset3
228554	10	421320	7	NULL	NULL	0	NULL	middle phenyl 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the lipophilicity and steric bulk of the terminal ring system , the amount of pi-electron density in the terminal ring , and the relative spatial proximity of the tetrazolyl and the middle phenyl are explored in terms of binding affinity to AT1 receptors in rat adrenal glomerulosa and rabbit aorta .
	manualset3
228555	11	421320	7	NULL	NULL	0	NULL	terms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the lipophilicity and steric bulk of the terminal ring system , the amount of pi-electron density in the terminal ring , and the relative spatial proximity of the tetrazolyl and the middle phenyl are explored in terms of binding affinity to AT1 receptors in rat adrenal glomerulosa and rabbit aorta .
	manualset3
228556	12	421320	7	NULL	NULL	0	NULL	binding affinity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the lipophilicity and steric bulk of the terminal ring system , the amount of pi-electron density in the terminal ring , and the relative spatial proximity of the tetrazolyl and the middle phenyl are explored in terms of binding affinity to AT1 receptors in rat adrenal glomerulosa and rabbit aorta .
	manualset3
228557	13	421320	7	NULL	NULL	0	NULL	AT1 receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the lipophilicity and steric bulk of the terminal ring system , the amount of pi-electron density in the terminal ring , and the relative spatial proximity of the tetrazolyl and the middle phenyl are explored in terms of binding affinity to AT1 receptors in rat adrenal glomerulosa and rabbit aorta .
	manualset3
228558	14	421320	7	NULL	NULL	0	NULL	rat adrenal glomerulosa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the lipophilicity and steric bulk of the terminal ring system , the amount of pi-electron density in the terminal ring , and the relative spatial proximity of the tetrazolyl and the middle phenyl are explored in terms of binding affinity to AT1 receptors in rat adrenal glomerulosa and rabbit aorta .
	manualset3
228559	15	421320	7	NULL	NULL	0	NULL	rabbit aorta 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of the lipophilicity and steric bulk of the terminal ring system , the amount of pi-electron density in the terminal ring , and the relative spatial proximity of the tetrazolyl and the middle phenyl are explored in terms of binding affinity to AT1 receptors in rat adrenal glomerulosa and rabbit aorta .
	manualset3
228587	1	421321	7	NULL	NULL	0	NULL	groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In all groups classified by the etiology , the causes of death had the same order in incidence .
	manualset3
228588	2	421321	7	NULL	NULL	0	NULL	etiology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In all groups classified by the etiology , the causes of death had the same order in incidence .
	manualset3
228589	3	421321	7	NULL	NULL	0	NULL	causes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In all groups classified by the etiology , the causes of death had the same order in incidence .
	manualset3
228590	4	421321	7	NULL	NULL	0	NULL	death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In all groups classified by the etiology , the causes of death had the same order in incidence .
	manualset3
228591	5	421321	7	NULL	NULL	0	NULL	order	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In all groups classified by the etiology , the causes of death had the same order in incidence .
	manualset3
228592	6	421321	7	NULL	NULL	0	NULL	incidence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In all groups classified by the etiology , the causes of death had the same order in incidence .
	manualset3
228593	1	421322	7	NULL	NULL	0	NULL	In vivo validation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo validation of MR velocity imaging .
	manualset3
228594	2	421322	7	NULL	NULL	0	NULL	MR velocity imaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In vivo validation of MR velocity imaging .
	manualset3
228595	1	421323	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the third experiment indicated that cusp calcification , which decreased significantly after a 12-month storage period , was reset to high levels by reexposing the valves to glutaraldehyde at the end of the 12-month storage period .
	manualset3
228596	2	421323	7	NULL	NULL	0	NULL	 third experiment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the third experiment indicated that cusp calcification , which decreased significantly after a 12-month storage period , was reset to high levels by reexposing the valves to glutaraldehyde at the end of the 12-month storage period .
	manualset3
228597	3	421323	7	NULL	NULL	0	NULL	cusp calcification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the third experiment indicated that cusp calcification , which decreased significantly after a 12-month storage period , was reset to high levels by reexposing the valves to glutaraldehyde at the end of the 12-month storage period .
	manualset3
228598	4	421323	7	NULL	NULL	0	NULL	12-month storage period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the third experiment indicated that cusp calcification , which decreased significantly after a 12-month storage period , was reset to high levels by reexposing the valves to glutaraldehyde at the end of the 12-month storage period .
	manualset3
228599	5	421323	7	NULL	NULL	0	NULL	 high levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the third experiment indicated that cusp calcification , which decreased significantly after a 12-month storage period , was reset to high levels by reexposing the valves to glutaraldehyde at the end of the 12-month storage period .
	manualset3
228600	6	421323	7	NULL	NULL	0	NULL	valves	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the third experiment indicated that cusp calcification , which decreased significantly after a 12-month storage period , was reset to high levels by reexposing the valves to glutaraldehyde at the end of the 12-month storage period .
	manualset3
228601	7	421323	7	NULL	NULL	0	NULL	glutaraldehyde	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the third experiment indicated that cusp calcification , which decreased significantly after a 12-month storage period , was reset to high levels by reexposing the valves to glutaraldehyde at the end of the 12-month storage period .
	manualset3
228602	8	421323	7	NULL	NULL	0	NULL	 end	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the third experiment indicated that cusp calcification , which decreased significantly after a 12-month storage period , was reset to high levels by reexposing the valves to glutaraldehyde at the end of the 12-month storage period .
	manualset3
228603	9	421323	7	NULL	NULL	0	NULL	12-month storage period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of the third experiment indicated that cusp calcification , which decreased significantly after a 12-month storage period , was reset to high levels by reexposing the valves to glutaraldehyde at the end of the 12-month storage period .
	manualset3
228604	1	421324	7	NULL	NULL	0	NULL	Amiodarone drug interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Amiodarone drug interactions : potential beneficial and adverse effects .
	manualset3
228605	4	421324	7	NULL	NULL	NULL	NULL	adverse effects 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Amiodarone drug interactions : potential beneficial and adverse effects .
	manualset3
229412	2	421324	7	NULL	NULL	NULL	NULL	potential effects	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Amiodarone drug interactions : potential beneficial and adverse effects .
	manualset3
229413	3	421324	7	NULL	NULL	0	NULL	beneficial effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Amiodarone drug interactions : potential beneficial and adverse effects .
	manualset3
228606	1	421325	7	NULL	NULL	0	NULL	lead compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This lead compound and its phosphate pro-drug have potent in vivo antimalarial activity after oral administration , consistent with the target product profile of a drug for the treatment of uncomplicated malaria .
	manualset3
228607	2	421325	7	NULL	NULL	0	NULL	phosphate pro-drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	This lead compound and its phosphate pro-drug have potent in vivo antimalarial activity after oral administration , consistent with the target product profile of a drug for the treatment of uncomplicated malaria .
	manualset3
228608	3	421325	7	NULL	NULL	0	NULL	in vivo antimalarial activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This lead compound and its phosphate pro-drug have potent in vivo antimalarial activity after oral administration , consistent with the target product profile of a drug for the treatment of uncomplicated malaria .
	manualset3
228609	4	421325	7	NULL	NULL	0	NULL	oral administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This lead compound and its phosphate pro-drug have potent in vivo antimalarial activity after oral administration , consistent with the target product profile of a drug for the treatment of uncomplicated malaria .
	manualset3
228610	5	421325	7	NULL	NULL	0	NULL	target product profile	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This lead compound and its phosphate pro-drug have potent in vivo antimalarial activity after oral administration , consistent with the target product profile of a drug for the treatment of uncomplicated malaria .
	manualset3
228611	6	421325	7	NULL	NULL	0	NULL	drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	This lead compound and its phosphate pro-drug have potent in vivo antimalarial activity after oral administration , consistent with the target product profile of a drug for the treatment of uncomplicated malaria .
	manualset3
228612	7	421325	7	NULL	NULL	0	NULL	 treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This lead compound and its phosphate pro-drug have potent in vivo antimalarial activity after oral administration , consistent with the target product profile of a drug for the treatment of uncomplicated malaria .
	manualset3
228613	8	421325	7	NULL	NULL	0	NULL	uncomplicated malaria	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This lead compound and its phosphate pro-drug have potent in vivo antimalarial activity after oral administration , consistent with the target product profile of a drug for the treatment of uncomplicated malaria .
	manualset3
228614	1	421326	7	NULL	NULL	0	NULL	12 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 12 patients with encapsulated thymic tumors the long term results were similar to those in patients with myasthenia gravis , whereas in patients with infiltrating thymic tumors the results were unsatisfactory .
	manualset3
228615	2	421326	7	NULL	NULL	0	NULL	encapsulated thymic tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In 12 patients with encapsulated thymic tumors the long term results were similar to those in patients with myasthenia gravis , whereas in patients with infiltrating thymic tumors the results were unsatisfactory .
	manualset3
228616	3	421326	7	NULL	NULL	0	NULL	long term results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 12 patients with encapsulated thymic tumors the long term results were similar to those in patients with myasthenia gravis , whereas in patients with infiltrating thymic tumors the results were unsatisfactory .
	manualset3
228617	4	421326	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 12 patients with encapsulated thymic tumors the long term results were similar to those in patients with myasthenia gravis , whereas in patients with infiltrating thymic tumors the results were unsatisfactory .
	manualset3
228618	5	421326	7	NULL	NULL	0	NULL	myasthenia gravis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In 12 patients with encapsulated thymic tumors the long term results were similar to those in patients with myasthenia gravis , whereas in patients with infiltrating thymic tumors the results were unsatisfactory .
	manualset3
228619	6	421326	7	NULL	NULL	0	NULL	 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 12 patients with encapsulated thymic tumors the long term results were similar to those in patients with myasthenia gravis , whereas in patients with infiltrating thymic tumors the results were unsatisfactory .
	manualset3
228620	7	421326	7	NULL	NULL	0	NULL	infiltrating thymic tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In 12 patients with encapsulated thymic tumors the long term results were similar to those in patients with myasthenia gravis , whereas in patients with infiltrating thymic tumors the results were unsatisfactory .
	manualset3
228621	8	421326	7	NULL	NULL	0	NULL	 results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 12 patients with encapsulated thymic tumors the long term results were similar to those in patients with myasthenia gravis , whereas in patients with infiltrating thymic tumors the results were unsatisfactory .
	manualset3
228622	1	421327	7	NULL	NULL	0	NULL	phytohemagglutinin ( PHA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	When cultured with phytohemagglutinin ( PHA ) , 90 % of the small cells underwent transformation , and they were found to be lymphoblast-like cells with irregular nuclei by electron microscopy .
	manualset3
228623	2	421327	7	NULL	NULL	0	NULL	90 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When cultured with phytohemagglutinin ( PHA ) , 90 % of the small cells underwent transformation , and they were found to be lymphoblast-like cells with irregular nuclei by electron microscopy .
	manualset3
228624	3	421327	7	NULL	NULL	0	NULL	small cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	When cultured with phytohemagglutinin ( PHA ) , 90 % of the small cells underwent transformation , and they were found to be lymphoblast-like cells with irregular nuclei by electron microscopy .
	manualset3
228625	4	421327	7	NULL	NULL	0	NULL	 transformation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When cultured with phytohemagglutinin ( PHA ) , 90 % of the small cells underwent transformation , and they were found to be lymphoblast-like cells with irregular nuclei by electron microscopy .
	manualset3
228626	5	421327	7	NULL	NULL	0	NULL	 lymphoblast-like cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	When cultured with phytohemagglutinin ( PHA ) , 90 % of the small cells underwent transformation , and they were found to be lymphoblast-like cells with irregular nuclei by electron microscopy .
	manualset3
228627	6	421327	7	NULL	NULL	0	NULL	 irregular nuclei	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	When cultured with phytohemagglutinin ( PHA ) , 90 % of the small cells underwent transformation , and they were found to be lymphoblast-like cells with irregular nuclei by electron microscopy .
	manualset3
228628	7	421327	7	NULL	NULL	0	NULL	electron microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	When cultured with phytohemagglutinin ( PHA ) , 90 % of the small cells underwent transformation , and they were found to be lymphoblast-like cells with irregular nuclei by electron microscopy .
	manualset3
228629	1	421328	7	NULL	NULL	0	NULL	 ill-posedness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Because of the ill-posedness , the inverse problem of BLT is still open .
	manualset3
228630	2	421328	7	NULL	NULL	0	NULL	 inverse problem 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Because of the ill-posedness , the inverse problem of BLT is still open .
	manualset3
228631	3	421328	7	NULL	NULL	0	NULL	BLT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Because of the ill-posedness , the inverse problem of BLT is still open .
	manualset3
228632	1	421329	7	NULL	NULL	0	NULL	Envirojet turfgrass injector	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An Envirojet turfgrass injector used to inject isazofos at 1.15 kg a.i. / ha and 2.88 kg a.i. / ha at 3 , 000 psi ( 1.38 x 107 Pascals ) significantly reduced nematode populations at 7 days after treatment at the low rate and at 63 days after treatment with both application rates .
	manualset3
228633	2	421329	7	NULL	NULL	0	NULL	isazofos	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An Envirojet turfgrass injector used to inject isazofos at 1.15 kg a.i. / ha and 2.88 kg a.i. / ha at 3 , 000 psi ( 1.38 x 107 Pascals ) significantly reduced nematode populations at 7 days after treatment at the low rate and at 63 days after treatment with both application rates .
	manualset3
228634	3	421329	7	NULL	NULL	0	NULL	 1.15 kg a.i. / ha	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An Envirojet turfgrass injector used to inject isazofos at 1.15 kg a.i. / ha and 2.88 kg a.i. / ha at 3 , 000 psi ( 1.38 x 107 Pascals ) significantly reduced nematode populations at 7 days after treatment at the low rate and at 63 days after treatment with both application rates .
	manualset3
228635	4	421329	7	NULL	NULL	0	NULL	2.88 kg a.i. / ha	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An Envirojet turfgrass injector used to inject isazofos at 1.15 kg a.i. / ha and 2.88 kg a.i. / ha at 3 , 000 psi ( 1.38 x 107 Pascals ) significantly reduced nematode populations at 7 days after treatment at the low rate and at 63 days after treatment with both application rates .
	manualset3
228636	5	421329	7	NULL	NULL	0	NULL	3 , 000 psi	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An Envirojet turfgrass injector used to inject isazofos at 1.15 kg a.i. / ha and 2.88 kg a.i. / ha at 3 , 000 psi ( 1.38 x 107 Pascals ) significantly reduced nematode populations at 7 days after treatment at the low rate and at 63 days after treatment with both application rates .
	manualset3
228637	6	421329	7	NULL	NULL	0	NULL	1.38 x 107 Pascals	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An Envirojet turfgrass injector used to inject isazofos at 1.15 kg a.i. / ha and 2.88 kg a.i. / ha at 3 , 000 psi ( 1.38 x 107 Pascals ) significantly reduced nematode populations at 7 days after treatment at the low rate and at 63 days after treatment with both application rates .
	manualset3
228638	7	421329	7	NULL	NULL	0	NULL	nematode populations	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	An Envirojet turfgrass injector used to inject isazofos at 1.15 kg a.i. / ha and 2.88 kg a.i. / ha at 3 , 000 psi ( 1.38 x 107 Pascals ) significantly reduced nematode populations at 7 days after treatment at the low rate and at 63 days after treatment with both application rates .
	manualset3
228639	8	421329	7	NULL	NULL	0	NULL	7 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	An Envirojet turfgrass injector used to inject isazofos at 1.15 kg a.i. / ha and 2.88 kg a.i. / ha at 3 , 000 psi ( 1.38 x 107 Pascals ) significantly reduced nematode populations at 7 days after treatment at the low rate and at 63 days after treatment with both application rates .
	manualset3
228640	9	421329	7	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An Envirojet turfgrass injector used to inject isazofos at 1.15 kg a.i. / ha and 2.88 kg a.i. / ha at 3 , 000 psi ( 1.38 x 107 Pascals ) significantly reduced nematode populations at 7 days after treatment at the low rate and at 63 days after treatment with both application rates .
	manualset3
228641	10	421329	7	NULL	NULL	0	NULL	low rate 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An Envirojet turfgrass injector used to inject isazofos at 1.15 kg a.i. / ha and 2.88 kg a.i. / ha at 3 , 000 psi ( 1.38 x 107 Pascals ) significantly reduced nematode populations at 7 days after treatment at the low rate and at 63 days after treatment with both application rates .
	manualset3
228642	11	421329	7	NULL	NULL	0	NULL	63 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	An Envirojet turfgrass injector used to inject isazofos at 1.15 kg a.i. / ha and 2.88 kg a.i. / ha at 3 , 000 psi ( 1.38 x 107 Pascals ) significantly reduced nematode populations at 7 days after treatment at the low rate and at 63 days after treatment with both application rates .
	manualset3
228643	12	421329	7	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An Envirojet turfgrass injector used to inject isazofos at 1.15 kg a.i. / ha and 2.88 kg a.i. / ha at 3 , 000 psi ( 1.38 x 107 Pascals ) significantly reduced nematode populations at 7 days after treatment at the low rate and at 63 days after treatment with both application rates .
	manualset3
228644	13	421329	7	NULL	NULL	0	NULL	application rates	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An Envirojet turfgrass injector used to inject isazofos at 1.15 kg a.i. / ha and 2.88 kg a.i. / ha at 3 , 000 psi ( 1.38 x 107 Pascals ) significantly reduced nematode populations at 7 days after treatment at the low rate and at 63 days after treatment with both application rates .
	manualset3
228645	1	421330	7	NULL	NULL	0	NULL	Proven antihepatotoxic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Proven antihepatotoxic activity of Sm can not therefore be fully exploited in acute chemical poisoning conditions like that in paracetamol overdose .
	manualset3
228646	2	421330	7	NULL	NULL	0	NULL	Sm 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Proven antihepatotoxic activity of Sm can not therefore be fully exploited in acute chemical poisoning conditions like that in paracetamol overdose .
	manualset3
228647	3	421330	7	NULL	NULL	0	NULL	acute chemical poisoning conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Proven antihepatotoxic activity of Sm can not therefore be fully exploited in acute chemical poisoning conditions like that in paracetamol overdose .
	manualset3
228648	4	421330	7	NULL	NULL	0	NULL	paracetamol overdose	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Proven antihepatotoxic activity of Sm can not therefore be fully exploited in acute chemical poisoning conditions like that in paracetamol overdose .
	manualset3
228707	1	421331	7	NULL	NULL	0	NULL	Lysozyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Lysozyme in the overall treatment of children with an influenza infection and pneumonia ) .
	manualset3
228708	2	421331	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Lysozyme in the overall treatment of children with an influenza infection and pneumonia ) .
	manualset3
228709	3	421331	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Lysozyme in the overall treatment of children with an influenza infection and pneumonia ) .
	manualset3
228710	4	421331	7	NULL	NULL	0	NULL	influenza infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Lysozyme in the overall treatment of children with an influenza infection and pneumonia ) .
	manualset3
228711	5	421331	7	NULL	NULL	0	NULL	pneumonia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Lysozyme in the overall treatment of children with an influenza infection and pneumonia ) .
	manualset3
228712	1	421332	7	NULL	NULL	0	NULL	 clinical course 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical course was characterized by abrupt onset and rapid progression of neurological signs and symptoms , which appeared to have responded quite well to prednisolone .
	manualset3
228713	2	421332	7	NULL	NULL	0	NULL	onset	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical course was characterized by abrupt onset and rapid progression of neurological signs and symptoms , which appeared to have responded quite well to prednisolone .
	manualset3
228714	3	421332	7	NULL	NULL	0	NULL	rapid progression 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical course was characterized by abrupt onset and rapid progression of neurological signs and symptoms , which appeared to have responded quite well to prednisolone .
	manualset3
228715	4	421332	7	NULL	NULL	0	NULL	neurological signs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical course was characterized by abrupt onset and rapid progression of neurological signs and symptoms , which appeared to have responded quite well to prednisolone .
	manualset3
228716	5	421332	7	NULL	NULL	0	NULL	symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical course was characterized by abrupt onset and rapid progression of neurological signs and symptoms , which appeared to have responded quite well to prednisolone .
	manualset3
228717	6	421332	7	NULL	NULL	0	NULL	prednisolone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The clinical course was characterized by abrupt onset and rapid progression of neurological signs and symptoms , which appeared to have responded quite well to prednisolone .
	manualset3
228718	1	421333	7	NULL	NULL	0	NULL	Pretreatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with low dose paliperidone or risperidone ( 0.01 mg/kg/day postnatal days 35-56 ) normalized prefrontal cortical basal extracellular glutamate ( p & lt ; 0.05 vs. poly I : C vehicle-treatment ) .
	manualset3
228719	2	421333	7	NULL	NULL	0	NULL	low dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with low dose paliperidone or risperidone ( 0.01 mg/kg/day postnatal days 35-56 ) normalized prefrontal cortical basal extracellular glutamate ( p & lt ; 0.05 vs. poly I : C vehicle-treatment ) .
	manualset3
228720	3	421333	7	NULL	NULL	0	NULL	paliperidone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with low dose paliperidone or risperidone ( 0.01 mg/kg/day postnatal days 35-56 ) normalized prefrontal cortical basal extracellular glutamate ( p & lt ; 0.05 vs. poly I : C vehicle-treatment ) .
	manualset3
228721	4	421333	7	NULL	NULL	0	NULL	risperidone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with low dose paliperidone or risperidone ( 0.01 mg/kg/day postnatal days 35-56 ) normalized prefrontal cortical basal extracellular glutamate ( p & lt ; 0.05 vs. poly I : C vehicle-treatment ) .
	manualset3
228722	5	421333	7	NULL	NULL	0	NULL	0.01 mg/kg/day	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with low dose paliperidone or risperidone ( 0.01 mg/kg/day postnatal days 35-56 ) normalized prefrontal cortical basal extracellular glutamate ( p & lt ; 0.05 vs. poly I : C vehicle-treatment ) .
	manualset3
228723	6	421333	7	NULL	NULL	0	NULL	postnatal days 35-56	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with low dose paliperidone or risperidone ( 0.01 mg/kg/day postnatal days 35-56 ) normalized prefrontal cortical basal extracellular glutamate ( p & lt ; 0.05 vs. poly I : C vehicle-treatment ) .
	manualset3
228724	7	421333	7	NULL	NULL	0	NULL	prefrontal cortical basal extracellular glutamate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with low dose paliperidone or risperidone ( 0.01 mg/kg/day postnatal days 35-56 ) normalized prefrontal cortical basal extracellular glutamate ( p & lt ; 0.05 vs. poly I : C vehicle-treatment ) .
	manualset3
228725	8	421333	7	NULL	NULL	0	NULL	p & lt	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with low dose paliperidone or risperidone ( 0.01 mg/kg/day postnatal days 35-56 ) normalized prefrontal cortical basal extracellular glutamate ( p & lt ; 0.05 vs. poly I : C vehicle-treatment ) .
	manualset3
228726	9	421333	7	NULL	NULL	0	NULL	 0.05 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with low dose paliperidone or risperidone ( 0.01 mg/kg/day postnatal days 35-56 ) normalized prefrontal cortical basal extracellular glutamate ( p & lt ; 0.05 vs. poly I : C vehicle-treatment ) .
	manualset3
228727	10	421333	7	NULL	NULL	0	NULL	poly I : C	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with low dose paliperidone or risperidone ( 0.01 mg/kg/day postnatal days 35-56 ) normalized prefrontal cortical basal extracellular glutamate ( p & lt ; 0.05 vs. poly I : C vehicle-treatment ) .
	manualset3
228728	11	421333	7	NULL	NULL	0	NULL	vehicle-treatment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pretreatment with low dose paliperidone or risperidone ( 0.01 mg/kg/day postnatal days 35-56 ) normalized prefrontal cortical basal extracellular glutamate ( p & lt ; 0.05 vs. poly I : C vehicle-treatment ) .
	manualset3
228729	1	421334	7	NULL	NULL	0	NULL	percentage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of positive specimens that contained normetabolite ( only ) ranged from 8.0 % for EDDP ( 2-ethylidene-1 , 5 - dimethyl-3 , 3 - diphenylpyrrolidine ) to 53.1 % for norpropoxyphene .
	manualset3
228730	2	421334	7	NULL	NULL	0	NULL	positive specimens	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of positive specimens that contained normetabolite ( only ) ranged from 8.0 % for EDDP ( 2-ethylidene-1 , 5 - dimethyl-3 , 3 - diphenylpyrrolidine ) to 53.1 % for norpropoxyphene .
	manualset3
228731	3	421334	7	NULL	NULL	0	NULL	normetabolite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of positive specimens that contained normetabolite ( only ) ranged from 8.0 % for EDDP ( 2-ethylidene-1 , 5 - dimethyl-3 , 3 - diphenylpyrrolidine ) to 53.1 % for norpropoxyphene .
	manualset3
228732	4	421334	7	NULL	NULL	0	NULL	 8.0 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of positive specimens that contained normetabolite ( only ) ranged from 8.0 % for EDDP ( 2-ethylidene-1 , 5 - dimethyl-3 , 3 - diphenylpyrrolidine ) to 53.1 % for norpropoxyphene .
	manualset3
228733	5	421334	7	NULL	NULL	0	NULL	EDDP ( 2-ethylidene-1 , 5 - dimethyl-3 , 3 - diphenylpyrrolidine )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of positive specimens that contained normetabolite ( only ) ranged from 8.0 % for EDDP ( 2-ethylidene-1 , 5 - dimethyl-3 , 3 - diphenylpyrrolidine ) to 53.1 % for norpropoxyphene .
	manualset3
228734	6	421334	7	NULL	NULL	0	NULL	53.1 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of positive specimens that contained normetabolite ( only ) ranged from 8.0 % for EDDP ( 2-ethylidene-1 , 5 - dimethyl-3 , 3 - diphenylpyrrolidine ) to 53.1 % for norpropoxyphene .
	manualset3
228735	7	421334	7	NULL	NULL	0	NULL	norpropoxyphene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentage of positive specimens that contained normetabolite ( only ) ranged from 8.0 % for EDDP ( 2-ethylidene-1 , 5 - dimethyl-3 , 3 - diphenylpyrrolidine ) to 53.1 % for norpropoxyphene .
	manualset3
228736	1	421335	7	NULL	NULL	NULL	NULL	perfusion ( washing )	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The perfusion ( washing ) of the abdominal cavity with isoosmomolar solution by I. I. Deryabin and M. N. Lizanets method following operations carried out upon 104 gynecological patients and 26 cases of Caesarean section was carried out .
	manualset3
228737	2	421335	7	NULL	NULL	0	NULL	 abdominal cavity	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The perfusion ( washing ) of the abdominal cavity with isoosmomolar solution by I. I. Deryabin and M. N. Lizanets method following operations carried out upon 104 gynecological patients and 26 cases of Caesarean section was carried out .
	manualset3
228738	3	421335	7	NULL	NULL	0	NULL	 isoosmomolar solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The perfusion ( washing ) of the abdominal cavity with isoosmomolar solution by I. I. Deryabin and M. N. Lizanets method following operations carried out upon 104 gynecological patients and 26 cases of Caesarean section was carried out .
	manualset3
228740	5	421335	7	NULL	NULL	NULL	NULL	I. I. Deryabin and M. N. Lizanets method 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The perfusion ( washing ) of the abdominal cavity with isoosmomolar solution by I. I. Deryabin and M. N. Lizanets method following operations carried out upon 104 gynecological patients and 26 cases of Caesarean section was carried out .
	manualset3
228741	6	421335	7	NULL	NULL	0	NULL	operations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The perfusion ( washing ) of the abdominal cavity with isoosmomolar solution by I. I. Deryabin and M. N. Lizanets method following operations carried out upon 104 gynecological patients and 26 cases of Caesarean section was carried out .
	manualset3
228742	7	421335	7	NULL	NULL	0	NULL	 104 gynecological patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The perfusion ( washing ) of the abdominal cavity with isoosmomolar solution by I. I. Deryabin and M. N. Lizanets method following operations carried out upon 104 gynecological patients and 26 cases of Caesarean section was carried out .
	manualset3
228743	8	421335	7	NULL	NULL	0	NULL	26 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The perfusion ( washing ) of the abdominal cavity with isoosmomolar solution by I. I. Deryabin and M. N. Lizanets method following operations carried out upon 104 gynecological patients and 26 cases of Caesarean section was carried out .
	manualset3
228744	9	421335	7	NULL	NULL	0	NULL	Caesarean section	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The perfusion ( washing ) of the abdominal cavity with isoosmomolar solution by I. I. Deryabin and M. N. Lizanets method following operations carried out upon 104 gynecological patients and 26 cases of Caesarean section was carried out .
	manualset3
228745	1	421336	7	NULL	NULL	0	NULL	review 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This review summarizes the results that help in understanding the role of morphine use in HIV infection and neural dysfunction .
	manualset3
228746	2	421336	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This review summarizes the results that help in understanding the role of morphine use in HIV infection and neural dysfunction .
	manualset3
228747	3	421336	7	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This review summarizes the results that help in understanding the role of morphine use in HIV infection and neural dysfunction .
	manualset3
228748	4	421336	7	NULL	NULL	0	NULL	morphine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	This review summarizes the results that help in understanding the role of morphine use in HIV infection and neural dysfunction .
	manualset3
228749	5	421336	7	NULL	NULL	0	NULL	 HIV infection	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This review summarizes the results that help in understanding the role of morphine use in HIV infection and neural dysfunction .
	manualset3
228750	6	421336	7	NULL	NULL	0	NULL	neural dysfunction	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This review summarizes the results that help in understanding the role of morphine use in HIV infection and neural dysfunction .
	manualset3
228751	1	421337	7	NULL	NULL	0	NULL	Exploration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An Exploration of the Discursive Constructions used in Young Adults ' Memories and Accounts of Contraception .
	manualset3
228752	2	421337	7	NULL	NULL	0	NULL	Discursive Constructions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An Exploration of the Discursive Constructions used in Young Adults ' Memories and Accounts of Contraception .
	manualset3
228753	3	421337	7	NULL	NULL	0	NULL	Young Adults ' Memories	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An Exploration of the Discursive Constructions used in Young Adults ' Memories and Accounts of Contraception .
	manualset3
228754	4	421337	7	NULL	NULL	NULL	NULL	Accounts 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An Exploration of the Discursive Constructions used in Young Adults ' Memories and Accounts of Contraception .
	manualset3
230482	5	421337	7	NULL	NULL	0	NULL	Contraception	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An Exploration of the Discursive Constructions used in Young Adults ' Memories and Accounts of Contraception .
	manualset3
228755	1	421338	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were divided into three groups according to their preservation scores .
	manualset3
228756	2	421338	7	NULL	NULL	0	NULL	three groups 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were divided into three groups according to their preservation scores .
	manualset3
228757	3	421338	7	NULL	NULL	0	NULL	preservation scores	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were divided into three groups according to their preservation scores .
	manualset3
228758	1	421339	7	NULL	NULL	0	NULL	selective and sensitive method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A selective and sensitive method for the determination of fenspiride in biological fluids is described .
	manualset3
228759	2	421339	7	NULL	NULL	0	NULL	determination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A selective and sensitive method for the determination of fenspiride in biological fluids is described .
	manualset3
228760	3	421339	7	NULL	NULL	0	NULL	fenspiride	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	A selective and sensitive method for the determination of fenspiride in biological fluids is described .
	manualset3
228761	4	421339	7	NULL	NULL	0	NULL	biological fluids	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A selective and sensitive method for the determination of fenspiride in biological fluids is described .
	manualset3
228762	1	421340	7	NULL	NULL	0	NULL	product	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The product of this reaction , mevalonic acid , is also a precursor of isoprenoids , molecules required for the activation of signalling G-proteins , such as Ras .
	manualset3
228763	2	421340	7	NULL	NULL	0	NULL	reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The product of this reaction , mevalonic acid , is also a precursor of isoprenoids , molecules required for the activation of signalling G-proteins , such as Ras .
	manualset3
228764	3	421340	7	NULL	NULL	0	NULL	mevalonic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The product of this reaction , mevalonic acid , is also a precursor of isoprenoids , molecules required for the activation of signalling G-proteins , such as Ras .
	manualset3
228765	4	421340	7	NULL	NULL	0	NULL	precursor	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The product of this reaction , mevalonic acid , is also a precursor of isoprenoids , molecules required for the activation of signalling G-proteins , such as Ras .
	manualset3
228766	5	421340	7	NULL	NULL	NULL	NULL	isoprenoids	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The product of this reaction , mevalonic acid , is also a precursor of isoprenoids , molecules required for the activation of signalling G-proteins , such as Ras .
	manualset3
228767	6	421340	7	NULL	NULL	0	NULL	molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The product of this reaction , mevalonic acid , is also a precursor of isoprenoids , molecules required for the activation of signalling G-proteins , such as Ras .
	manualset3
228768	7	421340	7	NULL	NULL	0	NULL	activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The product of this reaction , mevalonic acid , is also a precursor of isoprenoids , molecules required for the activation of signalling G-proteins , such as Ras .
	manualset3
228769	8	421340	7	NULL	NULL	0	NULL	signalling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The product of this reaction , mevalonic acid , is also a precursor of isoprenoids , molecules required for the activation of signalling G-proteins , such as Ras .
	manualset3
228770	9	421340	7	NULL	NULL	0	NULL	G-proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The product of this reaction , mevalonic acid , is also a precursor of isoprenoids , molecules required for the activation of signalling G-proteins , such as Ras .
	manualset3
228771	10	421340	7	NULL	NULL	0	NULL	Ras	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The product of this reaction , mevalonic acid , is also a precursor of isoprenoids , molecules required for the activation of signalling G-proteins , such as Ras .
	manualset3
228772	1	421341	7	NULL	NULL	0	NULL	change	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , a change in a child 's performance with a concomitant change in NAA and choline , as measured with magnetic resonance spectroscopy , could indicate the need for more aggressive intervention .
	manualset3
228773	2	421341	7	NULL	NULL	0	NULL	child 's performance	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , a change in a child 's performance with a concomitant change in NAA and choline , as measured with magnetic resonance spectroscopy , could indicate the need for more aggressive intervention .
	manualset3
228774	3	421341	7	NULL	NULL	0	NULL	concomitant change	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , a change in a child 's performance with a concomitant change in NAA and choline , as measured with magnetic resonance spectroscopy , could indicate the need for more aggressive intervention .
	manualset3
228775	4	421341	7	NULL	NULL	0	NULL	NAA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , a change in a child 's performance with a concomitant change in NAA and choline , as measured with magnetic resonance spectroscopy , could indicate the need for more aggressive intervention .
	manualset3
228776	5	421341	7	NULL	NULL	0	NULL	choline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , a change in a child 's performance with a concomitant change in NAA and choline , as measured with magnetic resonance spectroscopy , could indicate the need for more aggressive intervention .
	manualset3
228777	6	421341	7	NULL	NULL	0	NULL	magnetic resonance spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , a change in a child 's performance with a concomitant change in NAA and choline , as measured with magnetic resonance spectroscopy , could indicate the need for more aggressive intervention .
	manualset3
228778	7	421341	7	NULL	NULL	0	NULL	aggressive intervention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , a change in a child 's performance with a concomitant change in NAA and choline , as measured with magnetic resonance spectroscopy , could indicate the need for more aggressive intervention .
	manualset3
228779	1	421342	7	NULL	NULL	0	NULL	Lazaroid	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Lazaroid administered along with the LP diet prevented blood pressure elevation , enhanced vasomotor response to ANG II , impaired vasodilatation to sodium nitroprusside , and microvascular rarefaction in adult offspring .
	manualset3
228780	2	421342	7	NULL	NULL	0	NULL	LP diet 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Lazaroid administered along with the LP diet prevented blood pressure elevation , enhanced vasomotor response to ANG II , impaired vasodilatation to sodium nitroprusside , and microvascular rarefaction in adult offspring .
	manualset3
228781	3	421342	7	NULL	NULL	NULL	NULL	blood pressure elevation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Lazaroid administered along with the LP diet prevented blood pressure elevation , enhanced vasomotor response to ANG II , impaired vasodilatation to sodium nitroprusside , and microvascular rarefaction in adult offspring .
	manualset3
228782	4	421342	7	NULL	NULL	0	NULL	vasomotor response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lazaroid administered along with the LP diet prevented blood pressure elevation , enhanced vasomotor response to ANG II , impaired vasodilatation to sodium nitroprusside , and microvascular rarefaction in adult offspring .
	manualset3
228783	5	421342	7	NULL	NULL	0	NULL	ANG II 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Lazaroid administered along with the LP diet prevented blood pressure elevation , enhanced vasomotor response to ANG II , impaired vasodilatation to sodium nitroprusside , and microvascular rarefaction in adult offspring .
	manualset3
228784	6	421342	7	NULL	NULL	0	NULL	 impaired vasodilatation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lazaroid administered along with the LP diet prevented blood pressure elevation , enhanced vasomotor response to ANG II , impaired vasodilatation to sodium nitroprusside , and microvascular rarefaction in adult offspring .
	manualset3
228785	7	421342	7	NULL	NULL	0	NULL	sodium nitroprusside 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Lazaroid administered along with the LP diet prevented blood pressure elevation , enhanced vasomotor response to ANG II , impaired vasodilatation to sodium nitroprusside , and microvascular rarefaction in adult offspring .
	manualset3
228786	8	421342	7	NULL	NULL	0	NULL	microvascular rarefaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Lazaroid administered along with the LP diet prevented blood pressure elevation , enhanced vasomotor response to ANG II , impaired vasodilatation to sodium nitroprusside , and microvascular rarefaction in adult offspring .
	manualset3
228787	9	421342	7	NULL	NULL	0	NULL	adult offspring	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Lazaroid administered along with the LP diet prevented blood pressure elevation , enhanced vasomotor response to ANG II , impaired vasodilatation to sodium nitroprusside , and microvascular rarefaction in adult offspring .
	manualset3
228788	1	421343	7	NULL	NULL	NULL	NULL	two regioisomers 	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The two regioisomers of endohedral pyrrolidinodimetallofullerenes M ( 2 ) @ I ( h ) - C ( 80 ) ( CH ( 2 ) ) ( 2 ) NTrt ( M = La , Ce ; Trt = trityl ) were synthesized , isolated , and characterized .
	manualset3
228789	2	421343	7	NULL	NULL	0	NULL	endohedral pyrrolidinodimetallofullerenes M ( 2 ) @ I ( h ) - C ( 80 ) ( CH ( 2 ) ) ( 2 ) NTrt ( M = La , Ce ; Trt = trityl )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The two regioisomers of endohedral pyrrolidinodimetallofullerenes M ( 2 ) @ I ( h ) - C ( 80 ) ( CH ( 2 ) ) ( 2 ) NTrt ( M = La , Ce ; Trt = trityl ) were synthesized , isolated , and characterized .
	manualset3
228790	1	421344	7	NULL	NULL	0	NULL	 no significant differences	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Yet , there were no significant differences among those of PROH , DMSO and G ( p ) 0.05 , respectively ) .
	manualset3
228791	2	421344	7	NULL	NULL	0	NULL	PROH 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Yet , there were no significant differences among those of PROH , DMSO and G ( p ) 0.05 , respectively ) .
	manualset3
228792	3	421344	7	NULL	NULL	0	NULL	DMSO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Yet , there were no significant differences among those of PROH , DMSO and G ( p ) 0.05 , respectively ) .
	manualset3
228793	4	421344	7	NULL	NULL	0	NULL	G ( p ) 0.05 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Yet , there were no significant differences among those of PROH , DMSO and G ( p ) 0.05 , respectively ) .
	manualset3
228794	1	421345	7	NULL	NULL	0	NULL	 criteria	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Those who do not meet these criteria , however , should not be summarily refused surgery if they are willing to accept the possibility of an earlier death or prolonged disability over the certainty of a cancer-related death in the foreseeable months ahead .
	manualset3
228796	2	421345	7	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Those who do not meet these criteria , however , should not be summarily refused surgery if they are willing to accept the possibility of an earlier death or prolonged disability over the certainty of a cancer-related death in the foreseeable months ahead .
	manualset3
228797	3	421345	7	NULL	NULL	0	NULL	possibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Those who do not meet these criteria , however , should not be summarily refused surgery if they are willing to accept the possibility of an earlier death or prolonged disability over the certainty of a cancer-related death in the foreseeable months ahead .
	manualset3
228798	4	421345	7	NULL	NULL	0	NULL	 earlier death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Those who do not meet these criteria , however , should not be summarily refused surgery if they are willing to accept the possibility of an earlier death or prolonged disability over the certainty of a cancer-related death in the foreseeable months ahead .
	manualset3
228799	6	421345	7	NULL	NULL	NULL	NULL	cancer-related death 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Those who do not meet these criteria , however , should not be summarily refused surgery if they are willing to accept the possibility of an earlier death or prolonged disability over the certainty of a cancer-related death in the foreseeable months ahead .
	manualset3
228800	7	421345	7	NULL	NULL	NULL	NULL	foreseeable months	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Those who do not meet these criteria , however , should not be summarily refused surgery if they are willing to accept the possibility of an earlier death or prolonged disability over the certainty of a cancer-related death in the foreseeable months ahead .
	manualset3
228801	5	421345	7	NULL	NULL	0	NULL	prolonged disability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Those who do not meet these criteria , however , should not be summarily refused surgery if they are willing to accept the possibility of an earlier death or prolonged disability over the certainty of a cancer-related death in the foreseeable months ahead .
	manualset3
228802	1	421346	7	NULL	NULL	0	NULL	HPLC assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An HPLC assay for diclofenac ( DC ) and flurbiprofen ( FP ) in a 100-microliters sample of aqueous humor is presented .
	manualset3
228803	2	421346	7	NULL	NULL	0	NULL	 diclofenac ( DC ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	An HPLC assay for diclofenac ( DC ) and flurbiprofen ( FP ) in a 100-microliters sample of aqueous humor is presented .
	manualset3
228804	3	421346	7	NULL	NULL	0	NULL	flurbiprofen ( FP )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	An HPLC assay for diclofenac ( DC ) and flurbiprofen ( FP ) in a 100-microliters sample of aqueous humor is presented .
	manualset3
228805	4	421346	7	NULL	NULL	0	NULL	100-microliters sample	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	An HPLC assay for diclofenac ( DC ) and flurbiprofen ( FP ) in a 100-microliters sample of aqueous humor is presented .
	manualset3
228806	5	421346	7	NULL	NULL	0	NULL	aqueous humor	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An HPLC assay for diclofenac ( DC ) and flurbiprofen ( FP ) in a 100-microliters sample of aqueous humor is presented .
	manualset3
228807	1	421347	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Only one of two deaths was attributable to MRSA .
	manualset3
228808	2	421347	7	NULL	NULL	0	NULL	two deaths	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Only one of two deaths was attributable to MRSA .
	manualset3
228809	3	421347	7	NULL	NULL	0	NULL	MRSA	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Only one of two deaths was attributable to MRSA .
	manualset3
228810	1	421348	7	NULL	NULL	0	NULL	October 15 2010	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	On October 15 2010 the meeting ` Recombinant Pharmaceutical Manufacturing from Plants - The Future of Molecular Farming ' hosted by EuroScicon was held at BioPark Hertfordshire , Welwyn Garden city , UK .
	manualset3
228811	2	421348	7	NULL	NULL	0	NULL	meeting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On October 15 2010 the meeting ` Recombinant Pharmaceutical Manufacturing from Plants - The Future of Molecular Farming ' hosted by EuroScicon was held at BioPark Hertfordshire , Welwyn Garden city , UK .
	manualset3
228812	3	421348	7	NULL	NULL	NULL	NULL	Recombinant Pharmaceutical Manufacturing from Plants - The Future of Molecular Farming	PublicationOrCitation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On October 15 2010 the meeting ` Recombinant Pharmaceutical Manufacturing from Plants - The Future of Molecular Farming ' hosted by EuroScicon was held at BioPark Hertfordshire , Welwyn Garden city , UK .
	manualset3
228813	4	421348	7	NULL	NULL	0	NULL	EuroScicon	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	On October 15 2010 the meeting ` Recombinant Pharmaceutical Manufacturing from Plants - The Future of Molecular Farming ' hosted by EuroScicon was held at BioPark Hertfordshire , Welwyn Garden city , UK .
	manualset3
228814	5	421348	7	NULL	NULL	0	NULL	BioPark Hertfordshire	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	On October 15 2010 the meeting ` Recombinant Pharmaceutical Manufacturing from Plants - The Future of Molecular Farming ' hosted by EuroScicon was held at BioPark Hertfordshire , Welwyn Garden city , UK .
	manualset3
228815	6	421348	7	NULL	NULL	0	NULL	Welwyn Garden city	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	On October 15 2010 the meeting ` Recombinant Pharmaceutical Manufacturing from Plants - The Future of Molecular Farming ' hosted by EuroScicon was held at BioPark Hertfordshire , Welwyn Garden city , UK .
	manualset3
228816	7	421348	7	NULL	NULL	0	NULL	UK	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	On October 15 2010 the meeting ` Recombinant Pharmaceutical Manufacturing from Plants - The Future of Molecular Farming ' hosted by EuroScicon was held at BioPark Hertfordshire , Welwyn Garden city , UK .
	manualset3
228817	1	421349	7	NULL	NULL	0	NULL	Recommendation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Recommendation of the application of universal definition of myocardial infarction in China . ) .
	manualset3
228818	2	421349	7	NULL	NULL	0	NULL	application 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Recommendation of the application of universal definition of myocardial infarction in China . ) .
	manualset3
228819	3	421349	7	NULL	NULL	0	NULL	universal definition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Recommendation of the application of universal definition of myocardial infarction in China . ) .
	manualset3
228820	4	421349	7	NULL	NULL	0	NULL	myocardial infarction	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Recommendation of the application of universal definition of myocardial infarction in China . ) .
	manualset3
228821	5	421349	7	NULL	NULL	0	NULL	China 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Recommendation of the application of universal definition of myocardial infarction in China . ) .
	manualset3
228822	1	421350	7	NULL	NULL	0	NULL	AT cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	AT cells show dissimilar hypersensitivity to heavy-ion and X-rays irradiation .
	manualset3
228823	2	421350	7	NULL	NULL	0	NULL	dissimilar hypersensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	AT cells show dissimilar hypersensitivity to heavy-ion and X-rays irradiation .
	manualset3
228824	3	421350	7	NULL	NULL	0	NULL	heavy-ion  irradiation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	AT cells show dissimilar hypersensitivity to heavy-ion and X-rays irradiation .
	manualset3
228825	4	421350	7	NULL	NULL	0	NULL	 X-rays irradiation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	AT cells show dissimilar hypersensitivity to heavy-ion and X-rays irradiation .
	manualset3
228826	1	421351	7	NULL	NULL	0	NULL	clinically significant food interaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we were unable to detect any clinically significant food interaction , following ingestion of a quantity of cheese containing sufficient tyramine to increase systolic blood pressure by at least 30 mm Hg .
	manualset3
228827	2	421351	7	NULL	NULL	0	NULL	ingestion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we were unable to detect any clinically significant food interaction , following ingestion of a quantity of cheese containing sufficient tyramine to increase systolic blood pressure by at least 30 mm Hg .
	manualset3
228828	3	421351	7	NULL	NULL	0	NULL	quantity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we were unable to detect any clinically significant food interaction , following ingestion of a quantity of cheese containing sufficient tyramine to increase systolic blood pressure by at least 30 mm Hg .
	manualset3
228829	4	421351	7	NULL	NULL	0	NULL	 cheese	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we were unable to detect any clinically significant food interaction , following ingestion of a quantity of cheese containing sufficient tyramine to increase systolic blood pressure by at least 30 mm Hg .
	manualset3
228830	5	421351	7	NULL	NULL	0	NULL	tyramine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we were unable to detect any clinically significant food interaction , following ingestion of a quantity of cheese containing sufficient tyramine to increase systolic blood pressure by at least 30 mm Hg .
	manualset3
228831	6	421351	7	NULL	NULL	0	NULL	systolic blood pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we were unable to detect any clinically significant food interaction , following ingestion of a quantity of cheese containing sufficient tyramine to increase systolic blood pressure by at least 30 mm Hg .
	manualset3
228832	7	421351	7	NULL	NULL	0	NULL	30 mm Hg	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we were unable to detect any clinically significant food interaction , following ingestion of a quantity of cheese containing sufficient tyramine to increase systolic blood pressure by at least 30 mm Hg .
	manualset3
228833	1	421352	7	NULL	NULL	0	NULL	Extrahepatic portal venous obstruction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Extrahepatic portal venous obstruction : is the knife irrelevant ?
	manualset3
228834	2	421352	7	NULL	NULL	0	NULL	knife	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Extrahepatic portal venous obstruction : is the knife irrelevant ?
	manualset3
228835	1	421353	7	NULL	NULL	0	NULL	Superresolution microscopy techniques 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Superresolution microscopy techniques based on the sequential activation of fluorophores can achieve image resolution of 10nm but require a sparse distribution of simultaneously activated fluorophores in the field of view .
	manualset3
228836	2	421353	7	NULL	NULL	0	NULL	sequential activation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Superresolution microscopy techniques based on the sequential activation of fluorophores can achieve image resolution of 10nm but require a sparse distribution of simultaneously activated fluorophores in the field of view .
	manualset3
228837	3	421353	7	NULL	NULL	0	NULL	fluorophores	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Superresolution microscopy techniques based on the sequential activation of fluorophores can achieve image resolution of 10nm but require a sparse distribution of simultaneously activated fluorophores in the field of view .
	manualset3
228838	4	421353	7	NULL	NULL	0	NULL	image resolution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Superresolution microscopy techniques based on the sequential activation of fluorophores can achieve image resolution of 10nm but require a sparse distribution of simultaneously activated fluorophores in the field of view .
	manualset3
228839	5	421353	7	NULL	NULL	0	NULL	10nm	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Superresolution microscopy techniques based on the sequential activation of fluorophores can achieve image resolution of 10nm but require a sparse distribution of simultaneously activated fluorophores in the field of view .
	manualset3
228840	6	421353	7	NULL	NULL	0	NULL	sparse distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Superresolution microscopy techniques based on the sequential activation of fluorophores can achieve image resolution of 10nm but require a sparse distribution of simultaneously activated fluorophores in the field of view .
	manualset3
228841	7	421353	7	NULL	NULL	0	NULL	simultaneously activated fluorophores 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Superresolution microscopy techniques based on the sequential activation of fluorophores can achieve image resolution of 10nm but require a sparse distribution of simultaneously activated fluorophores in the field of view .
	manualset3
228842	8	421353	7	NULL	NULL	0	NULL	field of view	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Superresolution microscopy techniques based on the sequential activation of fluorophores can achieve image resolution of 10nm but require a sparse distribution of simultaneously activated fluorophores in the field of view .
	manualset3
228843	1	421354	7	NULL	NULL	0	NULL	Analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the MeC level in viral and cellular DNA obtained from mec ( + ) , mec ( + ) ( m ( N3 ) ( + ) ) , and mec ( - ) ( m ( N3 ) ( + ) ) strains has led to the conclusion that the R-factor controlled DNA-cytosine methylase may be capable of methylating a sequence ( s ) which is a substrate for the K-12 enzyme .
	manualset3
228844	2	421354	7	NULL	NULL	0	NULL	MeC level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the MeC level in viral and cellular DNA obtained from mec ( + ) , mec ( + ) ( m ( N3 ) ( + ) ) , and mec ( - ) ( m ( N3 ) ( + ) ) strains has led to the conclusion that the R-factor controlled DNA-cytosine methylase may be capable of methylating a sequence ( s ) which is a substrate for the K-12 enzyme .
	manualset3
228845	3	421354	7	NULL	NULL	0	NULL	viral DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the MeC level in viral and cellular DNA obtained from mec ( + ) , mec ( + ) ( m ( N3 ) ( + ) ) , and mec ( - ) ( m ( N3 ) ( + ) ) strains has led to the conclusion that the R-factor controlled DNA-cytosine methylase may be capable of methylating a sequence ( s ) which is a substrate for the K-12 enzyme .
	manualset3
228846	4	421354	7	NULL	NULL	0	NULL	cellular DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the MeC level in viral and cellular DNA obtained from mec ( + ) , mec ( + ) ( m ( N3 ) ( + ) ) , and mec ( - ) ( m ( N3 ) ( + ) ) strains has led to the conclusion that the R-factor controlled DNA-cytosine methylase may be capable of methylating a sequence ( s ) which is a substrate for the K-12 enzyme .
	manualset3
228847	5	421354	7	NULL	NULL	NULL	NULL	mec ( + ) strains	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Analysis of the MeC level in viral and cellular DNA obtained from mec ( + ) , mec ( + ) ( m ( N3 ) ( + ) ) , and mec ( - ) ( m ( N3 ) ( + ) ) strains has led to the conclusion that the R-factor controlled DNA-cytosine methylase may be capable of methylating a sequence ( s ) which is a substrate for the K-12 enzyme .
	manualset3
228848	6	421354	7	NULL	NULL	NULL	NULL	mec ( + )  ( m ( N3 ) ( + ) ) strains	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Analysis of the MeC level in viral and cellular DNA obtained from mec ( + ) , mec ( + ) ( m ( N3 ) ( + ) ) , and mec ( - ) ( m ( N3 ) ( + ) ) strains has led to the conclusion that the R-factor controlled DNA-cytosine methylase may be capable of methylating a sequence ( s ) which is a substrate for the K-12 enzyme .
	manualset3
228850	8	421354	7	NULL	NULL	0	NULL	mec ( - ) ( m ( N3 ) ( + ) ) strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the MeC level in viral and cellular DNA obtained from mec ( + ) , mec ( + ) ( m ( N3 ) ( + ) ) , and mec ( - ) ( m ( N3 ) ( + ) ) strains has led to the conclusion that the R-factor controlled DNA-cytosine methylase may be capable of methylating a sequence ( s ) which is a substrate for the K-12 enzyme .
	manualset3
228851	9	421354	7	NULL	NULL	0	NULL	conclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the MeC level in viral and cellular DNA obtained from mec ( + ) , mec ( + ) ( m ( N3 ) ( + ) ) , and mec ( - ) ( m ( N3 ) ( + ) ) strains has led to the conclusion that the R-factor controlled DNA-cytosine methylase may be capable of methylating a sequence ( s ) which is a substrate for the K-12 enzyme .
	manualset3
228852	10	421354	7	NULL	NULL	0	NULL	R-factor controlled DNA-cytosine methylase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the MeC level in viral and cellular DNA obtained from mec ( + ) , mec ( + ) ( m ( N3 ) ( + ) ) , and mec ( - ) ( m ( N3 ) ( + ) ) strains has led to the conclusion that the R-factor controlled DNA-cytosine methylase may be capable of methylating a sequence ( s ) which is a substrate for the K-12 enzyme .
	manualset3
228853	11	421354	7	NULL	NULL	0	NULL	sequence ( s )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the MeC level in viral and cellular DNA obtained from mec ( + ) , mec ( + ) ( m ( N3 ) ( + ) ) , and mec ( - ) ( m ( N3 ) ( + ) ) strains has led to the conclusion that the R-factor controlled DNA-cytosine methylase may be capable of methylating a sequence ( s ) which is a substrate for the K-12 enzyme .
	manualset3
228854	12	421354	7	NULL	NULL	0	NULL	substrate	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the MeC level in viral and cellular DNA obtained from mec ( + ) , mec ( + ) ( m ( N3 ) ( + ) ) , and mec ( - ) ( m ( N3 ) ( + ) ) strains has led to the conclusion that the R-factor controlled DNA-cytosine methylase may be capable of methylating a sequence ( s ) which is a substrate for the K-12 enzyme .
	manualset3
228855	13	421354	7	NULL	NULL	0	NULL	K-12 enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the MeC level in viral and cellular DNA obtained from mec ( + ) , mec ( + ) ( m ( N3 ) ( + ) ) , and mec ( - ) ( m ( N3 ) ( + ) ) strains has led to the conclusion that the R-factor controlled DNA-cytosine methylase may be capable of methylating a sequence ( s ) which is a substrate for the K-12 enzyme .
	manualset3
228856	1	421355	7	NULL	NULL	0	NULL	denied opportunities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We predicted that when denied opportunities for behavioural regulation , mobile , though brachypterous adults would show a performance advantage in most thermal environments following acclimation to their preferred temperature ( s ) .
	manualset3
228857	2	421355	7	NULL	NULL	0	NULL	behavioural regulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We predicted that when denied opportunities for behavioural regulation , mobile , though brachypterous adults would show a performance advantage in most thermal environments following acclimation to their preferred temperature ( s ) .
	manualset3
228858	3	421355	7	NULL	NULL	0	NULL	mobile	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	We predicted that when denied opportunities for behavioural regulation , mobile , though brachypterous adults would show a performance advantage in most thermal environments following acclimation to their preferred temperature ( s ) .
	manualset3
228859	4	421355	7	NULL	NULL	0	NULL	brachypterous adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We predicted that when denied opportunities for behavioural regulation , mobile , though brachypterous adults would show a performance advantage in most thermal environments following acclimation to their preferred temperature ( s ) .
	manualset3
228860	5	421355	7	NULL	NULL	0	NULL	performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We predicted that when denied opportunities for behavioural regulation , mobile , though brachypterous adults would show a performance advantage in most thermal environments following acclimation to their preferred temperature ( s ) .
	manualset3
228861	6	421355	7	NULL	NULL	0	NULL	thermal environments 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We predicted that when denied opportunities for behavioural regulation , mobile , though brachypterous adults would show a performance advantage in most thermal environments following acclimation to their preferred temperature ( s ) .
	manualset3
228862	7	421355	7	NULL	NULL	0	NULL	acclimation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We predicted that when denied opportunities for behavioural regulation , mobile , though brachypterous adults would show a performance advantage in most thermal environments following acclimation to their preferred temperature ( s ) .
	manualset3
228863	8	421355	7	NULL	NULL	0	NULL	preferred temperature ( s )	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We predicted that when denied opportunities for behavioural regulation , mobile , though brachypterous adults would show a performance advantage in most thermal environments following acclimation to their preferred temperature ( s ) .
	manualset3
228864	1	421356	7	NULL	NULL	0	NULL	Hereditary hypocomplementemia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hereditary hypocomplementemia of the third component of complement ( C3 ) was found in a strain of rabbits in which hereditary C8 alpha-gamma deficiency was also found .
	manualset3
228888	2	421356	7	NULL	NULL	0	NULL	third component 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hereditary hypocomplementemia of the third component of complement ( C3 ) was found in a strain of rabbits in which hereditary C8 alpha-gamma deficiency was also found .
	manualset3
228889	3	421356	7	NULL	NULL	0	NULL	complement ( C3 ) 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hereditary hypocomplementemia of the third component of complement ( C3 ) was found in a strain of rabbits in which hereditary C8 alpha-gamma deficiency was also found .
	manualset3
228890	4	421356	7	NULL	NULL	0	NULL	 strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hereditary hypocomplementemia of the third component of complement ( C3 ) was found in a strain of rabbits in which hereditary C8 alpha-gamma deficiency was also found .
	manualset3
228891	5	421356	7	NULL	NULL	0	NULL	 rabbits 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Hereditary hypocomplementemia of the third component of complement ( C3 ) was found in a strain of rabbits in which hereditary C8 alpha-gamma deficiency was also found .
	manualset3
228892	6	421356	7	NULL	NULL	0	NULL	hereditary C8 alpha-gamma deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hereditary hypocomplementemia of the third component of complement ( C3 ) was found in a strain of rabbits in which hereditary C8 alpha-gamma deficiency was also found .
	manualset3
228893	1	421357	7	NULL	NULL	0	NULL	 six patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We report six patients with the syndrome who were evaluated by a double-layer indirect immunofluorescence ( IF ) technic using patient serum and autologous lesional skin as substrate followed by conjugate .
	manualset3
228894	2	421357	7	NULL	NULL	0	NULL	syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We report six patients with the syndrome who were evaluated by a double-layer indirect immunofluorescence ( IF ) technic using patient serum and autologous lesional skin as substrate followed by conjugate .
	manualset3
228895	3	421357	7	NULL	NULL	0	NULL	double-layer indirect immunofluorescence ( IF ) technic 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We report six patients with the syndrome who were evaluated by a double-layer indirect immunofluorescence ( IF ) technic using patient serum and autologous lesional skin as substrate followed by conjugate .
	manualset3
228896	4	421357	7	NULL	NULL	0	NULL	patient serum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We report six patients with the syndrome who were evaluated by a double-layer indirect immunofluorescence ( IF ) technic using patient serum and autologous lesional skin as substrate followed by conjugate .
	manualset3
228897	5	421357	7	NULL	NULL	0	NULL	autologous lesional skin	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We report six patients with the syndrome who were evaluated by a double-layer indirect immunofluorescence ( IF ) technic using patient serum and autologous lesional skin as substrate followed by conjugate .
	manualset3
228898	6	421357	7	NULL	NULL	0	NULL	substrate 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We report six patients with the syndrome who were evaluated by a double-layer indirect immunofluorescence ( IF ) technic using patient serum and autologous lesional skin as substrate followed by conjugate .
	manualset3
228899	7	421357	7	NULL	NULL	0	NULL	 conjugate	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We report six patients with the syndrome who were evaluated by a double-layer indirect immunofluorescence ( IF ) technic using patient serum and autologous lesional skin as substrate followed by conjugate .
	manualset3
228900	1	421358	7	NULL	NULL	0	NULL	Calculation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Calculation of radioimmunochemical determinations by `` spline approximation '' ( author 's transl ) ) .
	manualset3
228901	2	421358	7	NULL	NULL	0	NULL	 radioimmunochemical determinations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Calculation of radioimmunochemical determinations by `` spline approximation '' ( author 's transl ) ) .
	manualset3
228902	3	421358	7	NULL	NULL	0	NULL	spline approximation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Calculation of radioimmunochemical determinations by `` spline approximation '' ( author 's transl ) ) .
	manualset3
228903	4	421358	7	NULL	NULL	0	NULL	author 's transl 	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Calculation of radioimmunochemical determinations by `` spline approximation '' ( author 's transl ) ) .
	manualset3
228904	1	421359	7	NULL	NULL	0	NULL	H.G. Wells 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	H.G. Wells , an enthusiastic admirer of Morris in the early days of the movement , became disillusioned as a result of the Malthusianism he learned from Huxley and his subsequent rejection of Lamarckism in light of Weismann 's experiments on mice .
	manualset3
228905	2	421359	7	NULL	NULL	0	NULL	enthusiastic admirer 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	H.G. Wells , an enthusiastic admirer of Morris in the early days of the movement , became disillusioned as a result of the Malthusianism he learned from Huxley and his subsequent rejection of Lamarckism in light of Weismann 's experiments on mice .
	manualset3
228906	3	421359	7	NULL	NULL	0	NULL	Morris	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	H.G. Wells , an enthusiastic admirer of Morris in the early days of the movement , became disillusioned as a result of the Malthusianism he learned from Huxley and his subsequent rejection of Lamarckism in light of Weismann 's experiments on mice .
	manualset3
228907	4	421359	7	NULL	NULL	0	NULL	early days 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	H.G. Wells , an enthusiastic admirer of Morris in the early days of the movement , became disillusioned as a result of the Malthusianism he learned from Huxley and his subsequent rejection of Lamarckism in light of Weismann 's experiments on mice .
	manualset3
228908	5	421359	7	NULL	NULL	0	NULL	movement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	H.G. Wells , an enthusiastic admirer of Morris in the early days of the movement , became disillusioned as a result of the Malthusianism he learned from Huxley and his subsequent rejection of Lamarckism in light of Weismann 's experiments on mice .
	manualset3
228909	6	421359	7	NULL	NULL	0	NULL	 result 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	H.G. Wells , an enthusiastic admirer of Morris in the early days of the movement , became disillusioned as a result of the Malthusianism he learned from Huxley and his subsequent rejection of Lamarckism in light of Weismann 's experiments on mice .
	manualset3
228910	7	421359	7	NULL	NULL	0	NULL	Malthusianism	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	H.G. Wells , an enthusiastic admirer of Morris in the early days of the movement , became disillusioned as a result of the Malthusianism he learned from Huxley and his subsequent rejection of Lamarckism in light of Weismann 's experiments on mice .
	manualset3
228911	8	421359	7	NULL	NULL	0	NULL	Huxley 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	H.G. Wells , an enthusiastic admirer of Morris in the early days of the movement , became disillusioned as a result of the Malthusianism he learned from Huxley and his subsequent rejection of Lamarckism in light of Weismann 's experiments on mice .
	manualset3
228912	9	421359	7	NULL	NULL	0	NULL	rejection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	H.G. Wells , an enthusiastic admirer of Morris in the early days of the movement , became disillusioned as a result of the Malthusianism he learned from Huxley and his subsequent rejection of Lamarckism in light of Weismann 's experiments on mice .
	manualset3
228913	10	421359	7	NULL	NULL	0	NULL	Lamarckism	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	H.G. Wells , an enthusiastic admirer of Morris in the early days of the movement , became disillusioned as a result of the Malthusianism he learned from Huxley and his subsequent rejection of Lamarckism in light of Weismann 's experiments on mice .
	manualset3
228914	11	421359	7	NULL	NULL	0	NULL	Weismann 's experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	H.G. Wells , an enthusiastic admirer of Morris in the early days of the movement , became disillusioned as a result of the Malthusianism he learned from Huxley and his subsequent rejection of Lamarckism in light of Weismann 's experiments on mice .
	manualset3
228915	12	421359	7	NULL	NULL	0	NULL	 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	H.G. Wells , an enthusiastic admirer of Morris in the early days of the movement , became disillusioned as a result of the Malthusianism he learned from Huxley and his subsequent rejection of Lamarckism in light of Weismann 's experiments on mice .
	manualset3
228916	1	421360	7	NULL	NULL	0	NULL	 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The mice in the early postnatal period were most sensitive to the life-shortening effect of radiation .
	manualset3
228917	2	421360	7	NULL	NULL	0	NULL	early postnatal period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The mice in the early postnatal period were most sensitive to the life-shortening effect of radiation .
	manualset3
228918	3	421360	7	NULL	NULL	0	NULL	life-shortening effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The mice in the early postnatal period were most sensitive to the life-shortening effect of radiation .
	manualset3
228919	4	421360	7	NULL	NULL	0	NULL	radiation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The mice in the early postnatal period were most sensitive to the life-shortening effect of radiation .
	manualset3
228920	1	421361	7	NULL	NULL	0	NULL	 Determination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of volatile compounds in biological media by gas chromatographic analysis of the equilibrium vapor phase ( review of the literature ) ) .
	manualset3
228921	2	421361	7	NULL	NULL	0	NULL	volatile compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of volatile compounds in biological media by gas chromatographic analysis of the equilibrium vapor phase ( review of the literature ) ) .
	manualset3
228922	3	421361	7	NULL	NULL	0	NULL	biological media	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of volatile compounds in biological media by gas chromatographic analysis of the equilibrium vapor phase ( review of the literature ) ) .
	manualset3
228923	4	421361	7	NULL	NULL	0	NULL	gas chromatographic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of volatile compounds in biological media by gas chromatographic analysis of the equilibrium vapor phase ( review of the literature ) ) .
	manualset3
228924	5	421361	7	NULL	NULL	0	NULL	equilibrium vapor phase	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of volatile compounds in biological media by gas chromatographic analysis of the equilibrium vapor phase ( review of the literature ) ) .
	manualset3
228925	6	421361	7	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of volatile compounds in biological media by gas chromatographic analysis of the equilibrium vapor phase ( review of the literature ) ) .
	manualset3
228926	7	421361	7	NULL	NULL	0	NULL	literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Determination of volatile compounds in biological media by gas chromatographic analysis of the equilibrium vapor phase ( review of the literature ) ) .
	manualset3
228927	1	421362	7	NULL	NULL	0	NULL	M cell model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	An M cell model has looser tight junctions than Caco-2 cells , but a similar level of particle uptake .
	manualset3
228928	2	421362	7	NULL	NULL	0	NULL	looser tight junctions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An M cell model has looser tight junctions than Caco-2 cells , but a similar level of particle uptake .
	manualset3
228929	3	421362	7	NULL	NULL	0	NULL	Caco-2 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	An M cell model has looser tight junctions than Caco-2 cells , but a similar level of particle uptake .
	manualset3
228930	4	421362	7	NULL	NULL	0	NULL	 similar level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An M cell model has looser tight junctions than Caco-2 cells , but a similar level of particle uptake .
	manualset3
228931	5	421362	7	NULL	NULL	0	NULL	particle uptake	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An M cell model has looser tight junctions than Caco-2 cells , but a similar level of particle uptake .
	manualset3
228932	1	421363	7	NULL	NULL	0	NULL	Subcellular fractionation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Subcellular fractionation and fluorescence microscopy revealed ALP transport defects in yck3Delta cells .
	manualset3
228933	2	421363	7	NULL	NULL	0	NULL	fluorescence microscopy 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Subcellular fractionation and fluorescence microscopy revealed ALP transport defects in yck3Delta cells .
	manualset3
228934	3	421363	7	NULL	NULL	0	NULL	ALP transport defects 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subcellular fractionation and fluorescence microscopy revealed ALP transport defects in yck3Delta cells .
	manualset3
228935	4	421363	7	NULL	NULL	0	NULL	yck3Delta cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Subcellular fractionation and fluorescence microscopy revealed ALP transport defects in yck3Delta cells .
	manualset3
228936	1	421364	7	NULL	NULL	0	NULL	Basic principles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Basic principles for the establishment of pharmacy network in various socialist countries ) .
	manualset3
228937	2	421364	7	NULL	NULL	0	NULL	establishment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Basic principles for the establishment of pharmacy network in various socialist countries ) .
	manualset3
228938	3	421364	7	NULL	NULL	0	NULL	pharmacy network	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( Basic principles for the establishment of pharmacy network in various socialist countries ) .
	manualset3
228939	4	421364	7	NULL	NULL	0	NULL	socialist countries	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Basic principles for the establishment of pharmacy network in various socialist countries ) .
	manualset3
228940	1	421365	7	NULL	NULL	0	NULL	restricted transformation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , the restricted transformation of human lymphocytes likely correlates with the specific SFK targeting by these oncoproteins .
	manualset3
228941	2	421365	7	NULL	NULL	0	NULL	human lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , the restricted transformation of human lymphocytes likely correlates with the specific SFK targeting by these oncoproteins .
	manualset3
228942	3	421365	7	NULL	NULL	0	NULL	specific SFK targeting	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , the restricted transformation of human lymphocytes likely correlates with the specific SFK targeting by these oncoproteins .
	manualset3
228943	4	421365	7	NULL	NULL	0	NULL	oncoproteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , the restricted transformation of human lymphocytes likely correlates with the specific SFK targeting by these oncoproteins .
	manualset3
228944	1	421366	7	NULL	NULL	0	NULL	factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Many factors may induce a reduction of the beta-cell function in patients with liver cirrhosis : some are due to a predisposition to the development of diabetes : genetic or environmental , unrelated to the hepatic disease ; some others are hepatic disease-dependent ( excess liver and islet of Langerhans iron deposition , HCV infection rather than other hepatic infections , the co-presence of HCC ) and may be crucial because additive to the previous .
	manualset3
228945	2	421366	7	NULL	NULL	0	NULL	reduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Many factors may induce a reduction of the beta-cell function in patients with liver cirrhosis : some are due to a predisposition to the development of diabetes : genetic or environmental , unrelated to the hepatic disease ; some others are hepatic disease-dependent ( excess liver and islet of Langerhans iron deposition , HCV infection rather than other hepatic infections , the co-presence of HCC ) and may be crucial because additive to the previous .
	manualset3
228946	3	421366	7	NULL	NULL	0	NULL	beta-cell function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Many factors may induce a reduction of the beta-cell function in patients with liver cirrhosis : some are due to a predisposition to the development of diabetes : genetic or environmental , unrelated to the hepatic disease ; some others are hepatic disease-dependent ( excess liver and islet of Langerhans iron deposition , HCV infection rather than other hepatic infections , the co-presence of HCC ) and may be crucial because additive to the previous .
	manualset3
228947	4	421366	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Many factors may induce a reduction of the beta-cell function in patients with liver cirrhosis : some are due to a predisposition to the development of diabetes : genetic or environmental , unrelated to the hepatic disease ; some others are hepatic disease-dependent ( excess liver and islet of Langerhans iron deposition , HCV infection rather than other hepatic infections , the co-presence of HCC ) and may be crucial because additive to the previous .
	manualset3
228948	5	421366	7	NULL	NULL	0	NULL	liver cirrhosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Many factors may induce a reduction of the beta-cell function in patients with liver cirrhosis : some are due to a predisposition to the development of diabetes : genetic or environmental , unrelated to the hepatic disease ; some others are hepatic disease-dependent ( excess liver and islet of Langerhans iron deposition , HCV infection rather than other hepatic infections , the co-presence of HCC ) and may be crucial because additive to the previous .
	manualset3
228949	6	421366	7	NULL	NULL	0	NULL	predisposition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many factors may induce a reduction of the beta-cell function in patients with liver cirrhosis : some are due to a predisposition to the development of diabetes : genetic or environmental , unrelated to the hepatic disease ; some others are hepatic disease-dependent ( excess liver and islet of Langerhans iron deposition , HCV infection rather than other hepatic infections , the co-presence of HCC ) and may be crucial because additive to the previous .
	manualset3
228950	7	421366	7	NULL	NULL	0	NULL	development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Many factors may induce a reduction of the beta-cell function in patients with liver cirrhosis : some are due to a predisposition to the development of diabetes : genetic or environmental , unrelated to the hepatic disease ; some others are hepatic disease-dependent ( excess liver and islet of Langerhans iron deposition , HCV infection rather than other hepatic infections , the co-presence of HCC ) and may be crucial because additive to the previous .
	manualset3
228951	8	421366	7	NULL	NULL	0	NULL	diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Many factors may induce a reduction of the beta-cell function in patients with liver cirrhosis : some are due to a predisposition to the development of diabetes : genetic or environmental , unrelated to the hepatic disease ; some others are hepatic disease-dependent ( excess liver and islet of Langerhans iron deposition , HCV infection rather than other hepatic infections , the co-presence of HCC ) and may be crucial because additive to the previous .
	manualset3
228952	9	421366	7	NULL	NULL	0	NULL	hepatic disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Many factors may induce a reduction of the beta-cell function in patients with liver cirrhosis : some are due to a predisposition to the development of diabetes : genetic or environmental , unrelated to the hepatic disease ; some others are hepatic disease-dependent ( excess liver and islet of Langerhans iron deposition , HCV infection rather than other hepatic infections , the co-presence of HCC ) and may be crucial because additive to the previous .
	manualset3
228953	10	421366	7	NULL	NULL	0	NULL	hepatic disease-dependent 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Many factors may induce a reduction of the beta-cell function in patients with liver cirrhosis : some are due to a predisposition to the development of diabetes : genetic or environmental , unrelated to the hepatic disease ; some others are hepatic disease-dependent ( excess liver and islet of Langerhans iron deposition , HCV infection rather than other hepatic infections , the co-presence of HCC ) and may be crucial because additive to the previous .
	manualset3
228954	11	421366	7	NULL	NULL	0	NULL	 liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Many factors may induce a reduction of the beta-cell function in patients with liver cirrhosis : some are due to a predisposition to the development of diabetes : genetic or environmental , unrelated to the hepatic disease ; some others are hepatic disease-dependent ( excess liver and islet of Langerhans iron deposition , HCV infection rather than other hepatic infections , the co-presence of HCC ) and may be crucial because additive to the previous .
	manualset3
228955	12	421366	7	NULL	NULL	0	NULL	 islet of Langerhans	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Many factors may induce a reduction of the beta-cell function in patients with liver cirrhosis : some are due to a predisposition to the development of diabetes : genetic or environmental , unrelated to the hepatic disease ; some others are hepatic disease-dependent ( excess liver and islet of Langerhans iron deposition , HCV infection rather than other hepatic infections , the co-presence of HCC ) and may be crucial because additive to the previous .
	manualset3
228956	13	421366	7	NULL	NULL	0	NULL	iron deposition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Many factors may induce a reduction of the beta-cell function in patients with liver cirrhosis : some are due to a predisposition to the development of diabetes : genetic or environmental , unrelated to the hepatic disease ; some others are hepatic disease-dependent ( excess liver and islet of Langerhans iron deposition , HCV infection rather than other hepatic infections , the co-presence of HCC ) and may be crucial because additive to the previous .
	manualset3
228957	14	421366	7	NULL	NULL	0	NULL	HCV infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Many factors may induce a reduction of the beta-cell function in patients with liver cirrhosis : some are due to a predisposition to the development of diabetes : genetic or environmental , unrelated to the hepatic disease ; some others are hepatic disease-dependent ( excess liver and islet of Langerhans iron deposition , HCV infection rather than other hepatic infections , the co-presence of HCC ) and may be crucial because additive to the previous .
	manualset3
228958	15	421366	7	NULL	NULL	0	NULL	hepatic infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Many factors may induce a reduction of the beta-cell function in patients with liver cirrhosis : some are due to a predisposition to the development of diabetes : genetic or environmental , unrelated to the hepatic disease ; some others are hepatic disease-dependent ( excess liver and islet of Langerhans iron deposition , HCV infection rather than other hepatic infections , the co-presence of HCC ) and may be crucial because additive to the previous .
	manualset3
228959	16	421366	7	NULL	NULL	0	NULL	co-presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Many factors may induce a reduction of the beta-cell function in patients with liver cirrhosis : some are due to a predisposition to the development of diabetes : genetic or environmental , unrelated to the hepatic disease ; some others are hepatic disease-dependent ( excess liver and islet of Langerhans iron deposition , HCV infection rather than other hepatic infections , the co-presence of HCC ) and may be crucial because additive to the previous .
	manualset3
228960	17	421366	7	NULL	NULL	0	NULL	HCC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Many factors may induce a reduction of the beta-cell function in patients with liver cirrhosis : some are due to a predisposition to the development of diabetes : genetic or environmental , unrelated to the hepatic disease ; some others are hepatic disease-dependent ( excess liver and islet of Langerhans iron deposition , HCV infection rather than other hepatic infections , the co-presence of HCC ) and may be crucial because additive to the previous .
	manualset3
228961	1	421367	7	NULL	NULL	0	NULL	in vitro studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent in vitro studies suggested that cAMP stimulates B-Raf/ERK activation and proliferation of cyst-derived cells in a Ca ( 2 + ) inhibitable , Ras-dependent manner .
	manualset3
228962	2	421367	7	NULL	NULL	0	NULL	cAMP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent in vitro studies suggested that cAMP stimulates B-Raf/ERK activation and proliferation of cyst-derived cells in a Ca ( 2 + ) inhibitable , Ras-dependent manner .
	manualset3
228963	3	421367	7	NULL	NULL	0	NULL	B-Raf/ERK activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent in vitro studies suggested that cAMP stimulates B-Raf/ERK activation and proliferation of cyst-derived cells in a Ca ( 2 + ) inhibitable , Ras-dependent manner .
	manualset3
228964	4	421367	7	NULL	NULL	0	NULL	proliferation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent in vitro studies suggested that cAMP stimulates B-Raf/ERK activation and proliferation of cyst-derived cells in a Ca ( 2 + ) inhibitable , Ras-dependent manner .
	manualset3
228965	5	421367	7	NULL	NULL	0	NULL	cyst-derived cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent in vitro studies suggested that cAMP stimulates B-Raf/ERK activation and proliferation of cyst-derived cells in a Ca ( 2 + ) inhibitable , Ras-dependent manner .
	manualset3
228966	6	421367	7	NULL	NULL	0	NULL	Ca ( 2 + ) inhibitable , Ras-dependent manner	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent in vitro studies suggested that cAMP stimulates B-Raf/ERK activation and proliferation of cyst-derived cells in a Ca ( 2 + ) inhibitable , Ras-dependent manner .
	manualset3
228967	1	421368	7	NULL	NULL	0	NULL	Block	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Block of FK1 was much more sensitive to pulse duration than was block of delta NCO , consistent with competition between N-type inactivation and 4-AP binding .
	manualset3
228968	2	421368	7	NULL	NULL	0	NULL	 FK1	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Block of FK1 was much more sensitive to pulse duration than was block of delta NCO , consistent with competition between N-type inactivation and 4-AP binding .
	manualset3
228969	3	421368	7	NULL	NULL	0	NULL	 pulse duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Block of FK1 was much more sensitive to pulse duration than was block of delta NCO , consistent with competition between N-type inactivation and 4-AP binding .
	manualset3
228970	4	421368	7	NULL	NULL	0	NULL	block	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Block of FK1 was much more sensitive to pulse duration than was block of delta NCO , consistent with competition between N-type inactivation and 4-AP binding .
	manualset3
228971	5	421368	7	NULL	NULL	0	NULL	 delta NCO	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Block of FK1 was much more sensitive to pulse duration than was block of delta NCO , consistent with competition between N-type inactivation and 4-AP binding .
	manualset3
228972	6	421368	7	NULL	NULL	0	NULL	competition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Block of FK1 was much more sensitive to pulse duration than was block of delta NCO , consistent with competition between N-type inactivation and 4-AP binding .
	manualset3
228973	7	421368	7	NULL	NULL	0	NULL	N-type inactivation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Block of FK1 was much more sensitive to pulse duration than was block of delta NCO , consistent with competition between N-type inactivation and 4-AP binding .
	manualset3
228974	8	421368	7	NULL	NULL	0	NULL	4-AP binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Block of FK1 was much more sensitive to pulse duration than was block of delta NCO , consistent with competition between N-type inactivation and 4-AP binding .
	manualset3
228975	1	421369	7	NULL	NULL	0	NULL	30 year old woman	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A 30 year old woman with primary hypothyroidism due to an ectopic ( sublingual ) thyroid , with a pituitary tumor invasive to the sphenoidal sinus presented with hyperprolactinemia , amenorrhoea and galactorrhoea not corrected by long-term thyroid replacement .
	manualset3
228976	2	421369	7	NULL	NULL	0	NULL	primary hypothyroidism	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A 30 year old woman with primary hypothyroidism due to an ectopic ( sublingual ) thyroid , with a pituitary tumor invasive to the sphenoidal sinus presented with hyperprolactinemia , amenorrhoea and galactorrhoea not corrected by long-term thyroid replacement .
	manualset3
228977	3	421369	7	NULL	NULL	0	NULL	ectopic ( sublingual ) thyroid	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A 30 year old woman with primary hypothyroidism due to an ectopic ( sublingual ) thyroid , with a pituitary tumor invasive to the sphenoidal sinus presented with hyperprolactinemia , amenorrhoea and galactorrhoea not corrected by long-term thyroid replacement .
	manualset3
228978	4	421369	7	NULL	NULL	0	NULL	pituitary tumor	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A 30 year old woman with primary hypothyroidism due to an ectopic ( sublingual ) thyroid , with a pituitary tumor invasive to the sphenoidal sinus presented with hyperprolactinemia , amenorrhoea and galactorrhoea not corrected by long-term thyroid replacement .
	manualset3
228979	5	421369	7	NULL	NULL	0	NULL	sphenoidal sinus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A 30 year old woman with primary hypothyroidism due to an ectopic ( sublingual ) thyroid , with a pituitary tumor invasive to the sphenoidal sinus presented with hyperprolactinemia , amenorrhoea and galactorrhoea not corrected by long-term thyroid replacement .
	manualset3
228980	6	421369	7	NULL	NULL	0	NULL	hyperprolactinemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A 30 year old woman with primary hypothyroidism due to an ectopic ( sublingual ) thyroid , with a pituitary tumor invasive to the sphenoidal sinus presented with hyperprolactinemia , amenorrhoea and galactorrhoea not corrected by long-term thyroid replacement .
	manualset3
228981	7	421369	7	NULL	NULL	0	NULL	amenorrhoea	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A 30 year old woman with primary hypothyroidism due to an ectopic ( sublingual ) thyroid , with a pituitary tumor invasive to the sphenoidal sinus presented with hyperprolactinemia , amenorrhoea and galactorrhoea not corrected by long-term thyroid replacement .
	manualset3
228982	8	421369	7	NULL	NULL	0	NULL	galactorrhoea 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A 30 year old woman with primary hypothyroidism due to an ectopic ( sublingual ) thyroid , with a pituitary tumor invasive to the sphenoidal sinus presented with hyperprolactinemia , amenorrhoea and galactorrhoea not corrected by long-term thyroid replacement .
	manualset3
228983	9	421369	7	NULL	NULL	0	NULL	long-term thyroid replacement 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A 30 year old woman with primary hypothyroidism due to an ectopic ( sublingual ) thyroid , with a pituitary tumor invasive to the sphenoidal sinus presented with hyperprolactinemia , amenorrhoea and galactorrhoea not corrected by long-term thyroid replacement .
	manualset3
228984	1	421370	7	NULL	NULL	0	NULL	genetic syndromes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Surprisingly , among the genetic syndromes associated to radiosensitivity there are some anomalies , not linked to DNA repair itself but to the intracellular trafficking .
	manualset3
228985	2	421370	7	NULL	NULL	0	NULL	radiosensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Surprisingly , among the genetic syndromes associated to radiosensitivity there are some anomalies , not linked to DNA repair itself but to the intracellular trafficking .
	manualset3
228986	3	421370	7	NULL	NULL	0	NULL	anomalies 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Surprisingly , among the genetic syndromes associated to radiosensitivity there are some anomalies , not linked to DNA repair itself but to the intracellular trafficking .
	manualset3
228987	4	421370	7	NULL	NULL	0	NULL	DNA repair	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Surprisingly , among the genetic syndromes associated to radiosensitivity there are some anomalies , not linked to DNA repair itself but to the intracellular trafficking .
	manualset3
228988	5	421370	7	NULL	NULL	0	NULL	intracellular trafficking	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Surprisingly , among the genetic syndromes associated to radiosensitivity there are some anomalies , not linked to DNA repair itself but to the intracellular trafficking .
	manualset3
228989	1	421371	7	NULL	NULL	0	NULL	day	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	By the day following completion of the treatment ( postnatal day 4 ) , degeneration of noradrenergic terminals in the parietal cortex and cerebellum was very extensive , with NE levels and DBH activities reduced by more than 80 % , and TOH activities reduced by 50 % .
	manualset3
228990	2	421371	7	NULL	NULL	0	NULL	completion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	By the day following completion of the treatment ( postnatal day 4 ) , degeneration of noradrenergic terminals in the parietal cortex and cerebellum was very extensive , with NE levels and DBH activities reduced by more than 80 % , and TOH activities reduced by 50 % .
	manualset3
228991	3	421371	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	By the day following completion of the treatment ( postnatal day 4 ) , degeneration of noradrenergic terminals in the parietal cortex and cerebellum was very extensive , with NE levels and DBH activities reduced by more than 80 % , and TOH activities reduced by 50 % .
	manualset3
228992	4	421371	7	NULL	NULL	0	NULL	postnatal day 4 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	By the day following completion of the treatment ( postnatal day 4 ) , degeneration of noradrenergic terminals in the parietal cortex and cerebellum was very extensive , with NE levels and DBH activities reduced by more than 80 % , and TOH activities reduced by 50 % .
	manualset3
228993	5	421371	7	NULL	NULL	0	NULL	 degeneration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	By the day following completion of the treatment ( postnatal day 4 ) , degeneration of noradrenergic terminals in the parietal cortex and cerebellum was very extensive , with NE levels and DBH activities reduced by more than 80 % , and TOH activities reduced by 50 % .
	manualset3
228994	6	421371	7	NULL	NULL	0	NULL	noradrenergic terminals	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	By the day following completion of the treatment ( postnatal day 4 ) , degeneration of noradrenergic terminals in the parietal cortex and cerebellum was very extensive , with NE levels and DBH activities reduced by more than 80 % , and TOH activities reduced by 50 % .
	manualset3
228995	7	421371	7	NULL	NULL	0	NULL	parietal cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	By the day following completion of the treatment ( postnatal day 4 ) , degeneration of noradrenergic terminals in the parietal cortex and cerebellum was very extensive , with NE levels and DBH activities reduced by more than 80 % , and TOH activities reduced by 50 % .
	manualset3
228996	8	421371	7	NULL	NULL	0	NULL	cerebellum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	By the day following completion of the treatment ( postnatal day 4 ) , degeneration of noradrenergic terminals in the parietal cortex and cerebellum was very extensive , with NE levels and DBH activities reduced by more than 80 % , and TOH activities reduced by 50 % .
	manualset3
228997	9	421371	7	NULL	NULL	0	NULL	NE levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	By the day following completion of the treatment ( postnatal day 4 ) , degeneration of noradrenergic terminals in the parietal cortex and cerebellum was very extensive , with NE levels and DBH activities reduced by more than 80 % , and TOH activities reduced by 50 % .
	manualset3
228998	10	421371	7	NULL	NULL	0	NULL	DBH activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	By the day following completion of the treatment ( postnatal day 4 ) , degeneration of noradrenergic terminals in the parietal cortex and cerebellum was very extensive , with NE levels and DBH activities reduced by more than 80 % , and TOH activities reduced by 50 % .
	manualset3
228999	11	421371	7	NULL	NULL	0	NULL	80 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	By the day following completion of the treatment ( postnatal day 4 ) , degeneration of noradrenergic terminals in the parietal cortex and cerebellum was very extensive , with NE levels and DBH activities reduced by more than 80 % , and TOH activities reduced by 50 % .
	manualset3
229000	12	421371	7	NULL	NULL	0	NULL	TOH activities 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	By the day following completion of the treatment ( postnatal day 4 ) , degeneration of noradrenergic terminals in the parietal cortex and cerebellum was very extensive , with NE levels and DBH activities reduced by more than 80 % , and TOH activities reduced by 50 % .
	manualset3
229001	13	421371	7	NULL	NULL	0	NULL	50 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	By the day following completion of the treatment ( postnatal day 4 ) , degeneration of noradrenergic terminals in the parietal cortex and cerebellum was very extensive , with NE levels and DBH activities reduced by more than 80 % , and TOH activities reduced by 50 % .
	manualset3
229002	1	421372	7	NULL	NULL	0	NULL	MPNST	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	An MPNST in such a location is very unusual .
	manualset3
229003	2	421372	7	NULL	NULL	0	NULL	location	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An MPNST in such a location is very unusual .
	manualset3
229004	1	421373	7	NULL	NULL	0	NULL	effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of ethylketocyclazocine ( EKC ) on the stereotyped behaviors induced by intraperitoneal injection of phencyclidine ( PCP ) or N-allylnormetazocine ( SKF 10 , 047 ) were examined .
	manualset3
229005	2	421373	7	NULL	NULL	0	NULL	ethylketocyclazocine ( EKC )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of ethylketocyclazocine ( EKC ) on the stereotyped behaviors induced by intraperitoneal injection of phencyclidine ( PCP ) or N-allylnormetazocine ( SKF 10 , 047 ) were examined .
	manualset3
229006	3	421373	7	NULL	NULL	0	NULL	stereotyped behaviors	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of ethylketocyclazocine ( EKC ) on the stereotyped behaviors induced by intraperitoneal injection of phencyclidine ( PCP ) or N-allylnormetazocine ( SKF 10 , 047 ) were examined .
	manualset3
229007	4	421373	7	NULL	NULL	0	NULL	intraperitoneal injection 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of ethylketocyclazocine ( EKC ) on the stereotyped behaviors induced by intraperitoneal injection of phencyclidine ( PCP ) or N-allylnormetazocine ( SKF 10 , 047 ) were examined .
	manualset3
229008	5	421373	7	NULL	NULL	0	NULL	phencyclidine ( PCP )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of ethylketocyclazocine ( EKC ) on the stereotyped behaviors induced by intraperitoneal injection of phencyclidine ( PCP ) or N-allylnormetazocine ( SKF 10 , 047 ) were examined .
	manualset3
229009	6	421373	7	NULL	NULL	0	NULL	N-allylnormetazocine ( SKF 10 , 047 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of ethylketocyclazocine ( EKC ) on the stereotyped behaviors induced by intraperitoneal injection of phencyclidine ( PCP ) or N-allylnormetazocine ( SKF 10 , 047 ) were examined .
	manualset3
229010	1	421374	7	NULL	NULL	0	NULL	Quantitative association	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative association between a newly identified molecular variant in the endothelin-2 gene and human essential hypertension .
	manualset3
229011	2	421374	7	NULL	NULL	0	NULL	newly identified molecular variant 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative association between a newly identified molecular variant in the endothelin-2 gene and human essential hypertension .
	manualset3
229012	3	421374	7	NULL	NULL	0	NULL	endothelin-2 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative association between a newly identified molecular variant in the endothelin-2 gene and human essential hypertension .
	manualset3
229013	4	421374	7	NULL	NULL	0	NULL	human essential hypertension	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Quantitative association between a newly identified molecular variant in the endothelin-2 gene and human essential hypertension .
	manualset3
229014	1	421375	7	NULL	NULL	0	NULL	scatter projections	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The scatter projections are generated by first forming an effective scatter source image ( ESSI ) , then forward-projecting the ESSI .
	manualset3
229015	2	421375	7	NULL	NULL	0	NULL	effective scatter source image ( ESSI )	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The scatter projections are generated by first forming an effective scatter source image ( ESSI ) , then forward-projecting the ESSI .
	manualset3
229016	3	421375	7	NULL	NULL	0	NULL	forward-projecting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The scatter projections are generated by first forming an effective scatter source image ( ESSI ) , then forward-projecting the ESSI .
	manualset3
229017	4	421375	7	NULL	NULL	0	NULL	ESSI	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The scatter projections are generated by first forming an effective scatter source image ( ESSI ) , then forward-projecting the ESSI .
	manualset3
229018	1	421376	7	NULL	NULL	0	NULL	Residents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Residents of Woburn were concerned over what they perceived to be a large number of childhood leukemia cases ; at the same time there was extensive publicity about uncontrolled hazardous waste sites in Woburn , which resulted in its being placed on the Superfund list .
	manualset3
229019	2	421376	7	NULL	NULL	0	NULL	Woburn 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Residents of Woburn were concerned over what they perceived to be a large number of childhood leukemia cases ; at the same time there was extensive publicity about uncontrolled hazardous waste sites in Woburn , which resulted in its being placed on the Superfund list .
	manualset3
229020	3	421376	7	NULL	NULL	0	NULL	 large number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Residents of Woburn were concerned over what they perceived to be a large number of childhood leukemia cases ; at the same time there was extensive publicity about uncontrolled hazardous waste sites in Woburn , which resulted in its being placed on the Superfund list .
	manualset3
229021	4	421376	7	NULL	NULL	0	NULL	childhood leukemia cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Residents of Woburn were concerned over what they perceived to be a large number of childhood leukemia cases ; at the same time there was extensive publicity about uncontrolled hazardous waste sites in Woburn , which resulted in its being placed on the Superfund list .
	manualset3
229022	5	421376	7	NULL	NULL	0	NULL	 time	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Residents of Woburn were concerned over what they perceived to be a large number of childhood leukemia cases ; at the same time there was extensive publicity about uncontrolled hazardous waste sites in Woburn , which resulted in its being placed on the Superfund list .
	manualset3
229023	6	421376	7	NULL	NULL	0	NULL	extensive publicity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Residents of Woburn were concerned over what they perceived to be a large number of childhood leukemia cases ; at the same time there was extensive publicity about uncontrolled hazardous waste sites in Woburn , which resulted in its being placed on the Superfund list .
	manualset3
229024	7	421376	7	NULL	NULL	0	NULL	uncontrolled hazardous waste sites	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Residents of Woburn were concerned over what they perceived to be a large number of childhood leukemia cases ; at the same time there was extensive publicity about uncontrolled hazardous waste sites in Woburn , which resulted in its being placed on the Superfund list .
	manualset3
229025	8	421376	7	NULL	NULL	0	NULL	Woburn	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Residents of Woburn were concerned over what they perceived to be a large number of childhood leukemia cases ; at the same time there was extensive publicity about uncontrolled hazardous waste sites in Woburn , which resulted in its being placed on the Superfund list .
	manualset3
229026	9	421376	7	NULL	NULL	0	NULL	 Superfund list	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Residents of Woburn were concerned over what they perceived to be a large number of childhood leukemia cases ; at the same time there was extensive publicity about uncontrolled hazardous waste sites in Woburn , which resulted in its being placed on the Superfund list .
	manualset3
229027	1	421377	7	NULL	NULL	0	NULL	N-methyl-D-aspartate ( NMDA ) receptor-mediated component 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	An N-methyl-D-aspartate ( NMDA ) receptor-mediated component of the unitary EPSP , elicited at the resting membrane potential in response to single action potentials in an individual CA3 cell , could be isolated pharmacologically .
	manualset3
229028	2	421377	7	NULL	NULL	0	NULL	unitary EPSP	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An N-methyl-D-aspartate ( NMDA ) receptor-mediated component of the unitary EPSP , elicited at the resting membrane potential in response to single action potentials in an individual CA3 cell , could be isolated pharmacologically .
	manualset3
229029	3	421377	7	NULL	NULL	0	NULL	resting membrane potential 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An N-methyl-D-aspartate ( NMDA ) receptor-mediated component of the unitary EPSP , elicited at the resting membrane potential in response to single action potentials in an individual CA3 cell , could be isolated pharmacologically .
	manualset3
229030	4	421377	7	NULL	NULL	0	NULL	single action potentials 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An N-methyl-D-aspartate ( NMDA ) receptor-mediated component of the unitary EPSP , elicited at the resting membrane potential in response to single action potentials in an individual CA3 cell , could be isolated pharmacologically .
	manualset3
229031	5	421377	7	NULL	NULL	0	NULL	individual CA3 cell 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	An N-methyl-D-aspartate ( NMDA ) receptor-mediated component of the unitary EPSP , elicited at the resting membrane potential in response to single action potentials in an individual CA3 cell , could be isolated pharmacologically .
	manualset3
230512	6	421377	7	NULL	NULL	0	NULL	response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An N-methyl-D-aspartate ( NMDA ) receptor-mediated component of the unitary EPSP , elicited at the resting membrane potential in response to single action potentials in an individual CA3 cell , could be isolated pharmacologically .
	manualset3
229032	1	421378	7	NULL	NULL	0	NULL	 basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These form the basis of a new library of computer programs , called ESTA ( Equilibrium Simulation for Titration Analysis ) .
	manualset3
229033	2	421378	7	NULL	NULL	0	NULL	new library 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	These form the basis of a new library of computer programs , called ESTA ( Equilibrium Simulation for Titration Analysis ) .
	manualset3
229034	3	421378	7	NULL	NULL	0	NULL	computer programs	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	These form the basis of a new library of computer programs , called ESTA ( Equilibrium Simulation for Titration Analysis ) .
	manualset3
229035	4	421378	7	NULL	NULL	0	NULL	ESTA ( Equilibrium Simulation for Titration Analysis )	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These form the basis of a new library of computer programs , called ESTA ( Equilibrium Simulation for Titration Analysis ) .
	manualset3
229036	1	421379	7	NULL	NULL	0	NULL	depolarization-induced transmembrane Ca2 + flux	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , depolarization-induced transmembrane Ca2 + flux was essential in securing the maintenance of the granule cells .
	manualset3
229037	2	421379	7	NULL	NULL	0	NULL	maintenance 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , depolarization-induced transmembrane Ca2 + flux was essential in securing the maintenance of the granule cells .
	manualset3
229038	3	421379	7	NULL	NULL	0	NULL	granule cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	On the other hand , depolarization-induced transmembrane Ca2 + flux was essential in securing the maintenance of the granule cells .
	manualset3
229039	1	421380	7	NULL	NULL	0	NULL	Anisodamine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Anisodamine in the treatment of 647 cases of severe hepatitis ) .
	manualset3
229040	2	421380	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Anisodamine in the treatment of 647 cases of severe hepatitis ) .
	manualset3
229041	3	421380	7	NULL	NULL	0	NULL	647 cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Anisodamine in the treatment of 647 cases of severe hepatitis ) .
	manualset3
229042	4	421380	7	NULL	NULL	0	NULL	severe hepatitis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Anisodamine in the treatment of 647 cases of severe hepatitis ) .
	manualset3
229043	1	421381	7	NULL	NULL	0	NULL	Adjuvant chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Adjuvant chemotherapy aimed at treating occult metastases .
	manualset3
229044	2	421381	7	NULL	NULL	0	NULL	 occult metastases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Adjuvant chemotherapy aimed at treating occult metastases .
	manualset3
229045	1	421382	7	NULL	NULL	0	NULL	cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In both cases , cells expressed large amounts of sialic acid , whereas they differed in their terminal nonreducing beta-D-galactosyl residues linked to N-acetyl galactosamine ; such residues were accessible to peanut agglutinin and Bauhinia purpurea lectin on cells grown in phorbol ester and inaccessible on cells grown with dialyzed hypothalamic extract .
	manualset3
229046	2	421382	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In both cases , cells expressed large amounts of sialic acid , whereas they differed in their terminal nonreducing beta-D-galactosyl residues linked to N-acetyl galactosamine ; such residues were accessible to peanut agglutinin and Bauhinia purpurea lectin on cells grown in phorbol ester and inaccessible on cells grown with dialyzed hypothalamic extract .
	manualset3
229047	3	421382	7	NULL	NULL	0	NULL	 large amounts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In both cases , cells expressed large amounts of sialic acid , whereas they differed in their terminal nonreducing beta-D-galactosyl residues linked to N-acetyl galactosamine ; such residues were accessible to peanut agglutinin and Bauhinia purpurea lectin on cells grown in phorbol ester and inaccessible on cells grown with dialyzed hypothalamic extract .
	manualset3
229048	4	421382	7	NULL	NULL	0	NULL	 sialic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In both cases , cells expressed large amounts of sialic acid , whereas they differed in their terminal nonreducing beta-D-galactosyl residues linked to N-acetyl galactosamine ; such residues were accessible to peanut agglutinin and Bauhinia purpurea lectin on cells grown in phorbol ester and inaccessible on cells grown with dialyzed hypothalamic extract .
	manualset3
229049	5	421382	7	NULL	NULL	0	NULL	 terminal nonreducing beta-D-galactosyl residues	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In both cases , cells expressed large amounts of sialic acid , whereas they differed in their terminal nonreducing beta-D-galactosyl residues linked to N-acetyl galactosamine ; such residues were accessible to peanut agglutinin and Bauhinia purpurea lectin on cells grown in phorbol ester and inaccessible on cells grown with dialyzed hypothalamic extract .
	manualset3
229050	6	421382	7	NULL	NULL	0	NULL	N-acetyl galactosamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In both cases , cells expressed large amounts of sialic acid , whereas they differed in their terminal nonreducing beta-D-galactosyl residues linked to N-acetyl galactosamine ; such residues were accessible to peanut agglutinin and Bauhinia purpurea lectin on cells grown in phorbol ester and inaccessible on cells grown with dialyzed hypothalamic extract .
	manualset3
229051	7	421382	7	NULL	NULL	0	NULL	 residues 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In both cases , cells expressed large amounts of sialic acid , whereas they differed in their terminal nonreducing beta-D-galactosyl residues linked to N-acetyl galactosamine ; such residues were accessible to peanut agglutinin and Bauhinia purpurea lectin on cells grown in phorbol ester and inaccessible on cells grown with dialyzed hypothalamic extract .
	manualset3
229052	8	421382	7	NULL	NULL	0	NULL	peanut agglutinin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In both cases , cells expressed large amounts of sialic acid , whereas they differed in their terminal nonreducing beta-D-galactosyl residues linked to N-acetyl galactosamine ; such residues were accessible to peanut agglutinin and Bauhinia purpurea lectin on cells grown in phorbol ester and inaccessible on cells grown with dialyzed hypothalamic extract .
	manualset3
229053	9	421382	7	NULL	NULL	0	NULL	Bauhinia purpurea lectin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In both cases , cells expressed large amounts of sialic acid , whereas they differed in their terminal nonreducing beta-D-galactosyl residues linked to N-acetyl galactosamine ; such residues were accessible to peanut agglutinin and Bauhinia purpurea lectin on cells grown in phorbol ester and inaccessible on cells grown with dialyzed hypothalamic extract .
	manualset3
229054	10	421382	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In both cases , cells expressed large amounts of sialic acid , whereas they differed in their terminal nonreducing beta-D-galactosyl residues linked to N-acetyl galactosamine ; such residues were accessible to peanut agglutinin and Bauhinia purpurea lectin on cells grown in phorbol ester and inaccessible on cells grown with dialyzed hypothalamic extract .
	manualset3
229055	11	421382	7	NULL	NULL	0	NULL	phorbol ester	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In both cases , cells expressed large amounts of sialic acid , whereas they differed in their terminal nonreducing beta-D-galactosyl residues linked to N-acetyl galactosamine ; such residues were accessible to peanut agglutinin and Bauhinia purpurea lectin on cells grown in phorbol ester and inaccessible on cells grown with dialyzed hypothalamic extract .
	manualset3
229056	12	421382	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In both cases , cells expressed large amounts of sialic acid , whereas they differed in their terminal nonreducing beta-D-galactosyl residues linked to N-acetyl galactosamine ; such residues were accessible to peanut agglutinin and Bauhinia purpurea lectin on cells grown in phorbol ester and inaccessible on cells grown with dialyzed hypothalamic extract .
	manualset3
229057	13	421382	7	NULL	NULL	0	NULL	dialyzed hypothalamic extract 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	In both cases , cells expressed large amounts of sialic acid , whereas they differed in their terminal nonreducing beta-D-galactosyl residues linked to N-acetyl galactosamine ; such residues were accessible to peanut agglutinin and Bauhinia purpurea lectin on cells grown in phorbol ester and inaccessible on cells grown with dialyzed hypothalamic extract .
	manualset3
229058	1	421383	7	NULL	NULL	NULL	NULL	Calcium score	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Calcium score as assessed by multi-slice computed tomography does not predict maximum plaque burden : an in vitro study .
	manualset3
229059	2	421383	7	NULL	NULL	0	NULL	multi-slice computed tomography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Calcium score as assessed by multi-slice computed tomography does not predict maximum plaque burden : an in vitro study .
	manualset3
229060	3	421383	7	NULL	NULL	0	NULL	maximum plaque burden	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Calcium score as assessed by multi-slice computed tomography does not predict maximum plaque burden : an in vitro study .
	manualset3
229061	4	421383	7	NULL	NULL	0	NULL	in vitro study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Calcium score as assessed by multi-slice computed tomography does not predict maximum plaque burden : an in vitro study .
	manualset3
229062	1	421384	7	NULL	NULL	0	NULL	 value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The value of serum biomarkers ( Bc1 , Bc2 , Bc3 ) in the diagnosis of early breast cancer .
	manualset3
229063	2	421384	7	NULL	NULL	0	NULL	serum biomarkers	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The value of serum biomarkers ( Bc1 , Bc2 , Bc3 ) in the diagnosis of early breast cancer .
	manualset3
229064	3	421384	7	NULL	NULL	NULL	NULL	Bc1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The value of serum biomarkers ( Bc1 , Bc2 , Bc3 ) in the diagnosis of early breast cancer .
	manualset3
229065	4	421384	7	NULL	NULL	0	NULL	Bc2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The value of serum biomarkers ( Bc1 , Bc2 , Bc3 ) in the diagnosis of early breast cancer .
	manualset3
229066	5	421384	7	NULL	NULL	0	NULL	Bc3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The value of serum biomarkers ( Bc1 , Bc2 , Bc3 ) in the diagnosis of early breast cancer .
	manualset3
229067	6	421384	7	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The value of serum biomarkers ( Bc1 , Bc2 , Bc3 ) in the diagnosis of early breast cancer .
	manualset3
229068	7	421384	7	NULL	NULL	0	NULL	early breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The value of serum biomarkers ( Bc1 , Bc2 , Bc3 ) in the diagnosis of early breast cancer .
	manualset3
229069	1	421385	7	NULL	NULL	0	NULL	 guidelines 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the most recent guidelines , low-density lipoprotein cholesterol ( LDLC ) is the principal target of lipid-lowering therapy and 3-hydroxy-3-methylglutaryl coenzyme A reductase inhibitors ( statins ) are the mainstay of this therapy .
	manualset3
229070	2	421385	7	NULL	NULL	0	NULL	low-density lipoprotein cholesterol ( LDLC )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the most recent guidelines , low-density lipoprotein cholesterol ( LDLC ) is the principal target of lipid-lowering therapy and 3-hydroxy-3-methylglutaryl coenzyme A reductase inhibitors ( statins ) are the mainstay of this therapy .
	manualset3
229071	3	421385	7	NULL	NULL	0	NULL	principal target	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the most recent guidelines , low-density lipoprotein cholesterol ( LDLC ) is the principal target of lipid-lowering therapy and 3-hydroxy-3-methylglutaryl coenzyme A reductase inhibitors ( statins ) are the mainstay of this therapy .
	manualset3
229072	4	421385	7	NULL	NULL	0	NULL	lipid-lowering therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the most recent guidelines , low-density lipoprotein cholesterol ( LDLC ) is the principal target of lipid-lowering therapy and 3-hydroxy-3-methylglutaryl coenzyme A reductase inhibitors ( statins ) are the mainstay of this therapy .
	manualset3
229073	5	421385	7	NULL	NULL	0	NULL	3-hydroxy-3-methylglutaryl coenzyme A reductase inhibitors ( statins ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the most recent guidelines , low-density lipoprotein cholesterol ( LDLC ) is the principal target of lipid-lowering therapy and 3-hydroxy-3-methylglutaryl coenzyme A reductase inhibitors ( statins ) are the mainstay of this therapy .
	manualset3
229074	6	421385	7	NULL	NULL	NULL	NULL	 mainstay 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	According to the most recent guidelines , low-density lipoprotein cholesterol ( LDLC ) is the principal target of lipid-lowering therapy and 3-hydroxy-3-methylglutaryl coenzyme A reductase inhibitors ( statins ) are the mainstay of this therapy .
	manualset3
229075	7	421385	7	NULL	NULL	0	NULL	 therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the most recent guidelines , low-density lipoprotein cholesterol ( LDLC ) is the principal target of lipid-lowering therapy and 3-hydroxy-3-methylglutaryl coenzyme A reductase inhibitors ( statins ) are the mainstay of this therapy .
	manualset3
229076	1	421386	7	NULL	NULL	0	NULL	abdominal x-ray	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An abdominal x-ray showed that the IUS was in the left hypochondrium .
	manualset3
229077	2	421386	7	NULL	NULL	0	NULL	 IUS	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	An abdominal x-ray showed that the IUS was in the left hypochondrium .
	manualset3
229078	3	421386	7	NULL	NULL	0	NULL	left hypochondrium 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An abdominal x-ray showed that the IUS was in the left hypochondrium .
	manualset3
229079	1	421387	7	NULL	NULL	0	NULL	Forensic-medical service 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( Forensic-medical service in Leningrad in the years before World War II and during the Blockade ) .
	manualset3
229080	2	421387	7	NULL	NULL	0	NULL	Leningrad	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Forensic-medical service in Leningrad in the years before World War II and during the Blockade ) .
	manualset3
229081	3	421387	7	NULL	NULL	0	NULL	years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	( Forensic-medical service in Leningrad in the years before World War II and during the Blockade ) .
	manualset3
229082	4	421387	7	NULL	NULL	0	NULL	World War II	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Forensic-medical service in Leningrad in the years before World War II and during the Blockade ) .
	manualset3
229083	5	421387	7	NULL	NULL	0	NULL	Blockade 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Forensic-medical service in Leningrad in the years before World War II and during the Blockade ) .
	manualset3
229084	1	421388	7	NULL	NULL	0	NULL	Analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of phosphorescence decay in heterogeneous systems : consequences of finite excitation flash duration .
	manualset3
229085	2	421388	7	NULL	NULL	0	NULL	phosphorescence decay	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of phosphorescence decay in heterogeneous systems : consequences of finite excitation flash duration .
	manualset3
229086	3	421388	7	NULL	NULL	0	NULL	heterogeneous systems	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of phosphorescence decay in heterogeneous systems : consequences of finite excitation flash duration .
	manualset3
229087	4	421388	7	NULL	NULL	0	NULL	consequences	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of phosphorescence decay in heterogeneous systems : consequences of finite excitation flash duration .
	manualset3
229088	5	421388	7	NULL	NULL	0	NULL	finite excitation flash duration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of phosphorescence decay in heterogeneous systems : consequences of finite excitation flash duration .
	manualset3
229089	1	421389	7	NULL	NULL	0	NULL	program	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The program uses scientific knowledge to estimate development indicators such as mortality , morbidity , fertility , school performance and labor productivity from the size and nutritional condition of populations .
	manualset3
229090	2	421389	7	NULL	NULL	0	NULL	scientific knowledge 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The program uses scientific knowledge to estimate development indicators such as mortality , morbidity , fertility , school performance and labor productivity from the size and nutritional condition of populations .
	manualset3
229091	3	421389	7	NULL	NULL	0	NULL	development indicators	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The program uses scientific knowledge to estimate development indicators such as mortality , morbidity , fertility , school performance and labor productivity from the size and nutritional condition of populations .
	manualset3
229092	4	421389	7	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The program uses scientific knowledge to estimate development indicators such as mortality , morbidity , fertility , school performance and labor productivity from the size and nutritional condition of populations .
	manualset3
229093	5	421389	7	NULL	NULL	0	NULL	morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The program uses scientific knowledge to estimate development indicators such as mortality , morbidity , fertility , school performance and labor productivity from the size and nutritional condition of populations .
	manualset3
229094	6	421389	7	NULL	NULL	0	NULL	fertility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The program uses scientific knowledge to estimate development indicators such as mortality , morbidity , fertility , school performance and labor productivity from the size and nutritional condition of populations .
	manualset3
229095	7	421389	7	NULL	NULL	0	NULL	school performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The program uses scientific knowledge to estimate development indicators such as mortality , morbidity , fertility , school performance and labor productivity from the size and nutritional condition of populations .
	manualset3
229096	8	421389	7	NULL	NULL	0	NULL	labor productivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The program uses scientific knowledge to estimate development indicators such as mortality , morbidity , fertility , school performance and labor productivity from the size and nutritional condition of populations .
	manualset3
229097	9	421389	7	NULL	NULL	0	NULL	size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The program uses scientific knowledge to estimate development indicators such as mortality , morbidity , fertility , school performance and labor productivity from the size and nutritional condition of populations .
	manualset3
229098	10	421389	7	NULL	NULL	0	NULL	nutritional condition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The program uses scientific knowledge to estimate development indicators such as mortality , morbidity , fertility , school performance and labor productivity from the size and nutritional condition of populations .
	manualset3
229099	11	421389	7	NULL	NULL	0	NULL	 populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The program uses scientific knowledge to estimate development indicators such as mortality , morbidity , fertility , school performance and labor productivity from the size and nutritional condition of populations .
	manualset3
229100	1	421390	7	NULL	NULL	0	NULL	modeling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The modeling of anticipatory coarticulation has been the subject of longstanding debates for more than 40 yr .
	manualset3
229101	2	421390	7	NULL	NULL	0	NULL	anticipatory coarticulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The modeling of anticipatory coarticulation has been the subject of longstanding debates for more than 40 yr .
	manualset3
229102	3	421390	7	NULL	NULL	0	NULL	subject 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The modeling of anticipatory coarticulation has been the subject of longstanding debates for more than 40 yr .
	manualset3
229103	4	421390	7	NULL	NULL	0	NULL	longstanding debates	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The modeling of anticipatory coarticulation has been the subject of longstanding debates for more than 40 yr .
	manualset3
229104	5	421390	7	NULL	NULL	0	NULL	40 yr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The modeling of anticipatory coarticulation has been the subject of longstanding debates for more than 40 yr .
	manualset3
229105	1	421391	7	NULL	NULL	0	NULL	Relative decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative decrease of IgM + IgD + cells at early phase was more profound in peritoneal cells ( PC ) than in spleen cells .
	manualset3
229106	2	421391	7	NULL	NULL	0	NULL	IgM + IgD + cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative decrease of IgM + IgD + cells at early phase was more profound in peritoneal cells ( PC ) than in spleen cells .
	manualset3
229107	3	421391	7	NULL	NULL	0	NULL	early phase	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative decrease of IgM + IgD + cells at early phase was more profound in peritoneal cells ( PC ) than in spleen cells .
	manualset3
229108	4	421391	7	NULL	NULL	0	NULL	peritoneal cells ( PC )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative decrease of IgM + IgD + cells at early phase was more profound in peritoneal cells ( PC ) than in spleen cells .
	manualset3
229109	5	421391	7	NULL	NULL	0	NULL	spleen cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Relative decrease of IgM + IgD + cells at early phase was more profound in peritoneal cells ( PC ) than in spleen cells .
	manualset3
229110	1	421392	7	NULL	NULL	0	NULL	112 identified articles	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 112 identified articles , 25 were selected for review .
	manualset3
229111	2	421392	7	NULL	NULL	0	NULL	25	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 112 identified articles , 25 were selected for review .
	manualset3
229112	3	421392	7	NULL	NULL	0	NULL	 review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 112 identified articles , 25 were selected for review .
	manualset3
229113	1	421393	7	NULL	NULL	0	NULL	 forested area	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	II ) situated in a forested area , a grass sports field and an orchard at a level of 1.5 million/m ( 2 ) .
	manualset3
229114	2	421393	7	NULL	NULL	0	NULL	grass sports field	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	II ) situated in a forested area , a grass sports field and an orchard at a level of 1.5 million/m ( 2 ) .
	manualset3
229115	3	421393	7	NULL	NULL	0	NULL	 orchard	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	II ) situated in a forested area , a grass sports field and an orchard at a level of 1.5 million/m ( 2 ) .
	manualset3
229116	4	421393	7	NULL	NULL	0	NULL	 level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	II ) situated in a forested area , a grass sports field and an orchard at a level of 1.5 million/m ( 2 ) .
	manualset3
229117	5	421393	7	NULL	NULL	0	NULL	1.5 million/m ( 2 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	II ) situated in a forested area , a grass sports field and an orchard at a level of 1.5 million/m ( 2 ) .
	manualset3
229118	1	421394	7	NULL	NULL	0	NULL	Prostate Cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Prostate Cancer : imaging , management , and screening .
	manualset3
229119	2	421394	7	NULL	NULL	0	NULL	imaging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prostate Cancer : imaging , management , and screening .
	manualset3
229120	3	421394	7	NULL	NULL	0	NULL	management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prostate Cancer : imaging , management , and screening .
	manualset3
229121	4	421394	7	NULL	NULL	0	NULL	screening 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Prostate Cancer : imaging , management , and screening .
	manualset3
229122	1	421395	7	NULL	NULL	0	NULL	Indications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Indications are that the reduced Na + content in derepressed cells inhibits Na + , K ( + ) - ATPase activity and that conditions that favored derepression do not allow for de novo synthesis of the Na + , K ( + ) - ATPase .
	manualset3
229123	2	421395	7	NULL	NULL	0	NULL	reduced Na + content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Indications are that the reduced Na + content in derepressed cells inhibits Na + , K ( + ) - ATPase activity and that conditions that favored derepression do not allow for de novo synthesis of the Na + , K ( + ) - ATPase .
	manualset3
229124	3	421395	7	NULL	NULL	0	NULL	derepressed cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Indications are that the reduced Na + content in derepressed cells inhibits Na + , K ( + ) - ATPase activity and that conditions that favored derepression do not allow for de novo synthesis of the Na + , K ( + ) - ATPase .
	manualset3
229125	4	421395	7	NULL	NULL	0	NULL	Na + , K ( + ) - ATPase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Indications are that the reduced Na + content in derepressed cells inhibits Na + , K ( + ) - ATPase activity and that conditions that favored derepression do not allow for de novo synthesis of the Na + , K ( + ) - ATPase .
	manualset3
229126	5	421395	7	NULL	NULL	0	NULL	conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Indications are that the reduced Na + content in derepressed cells inhibits Na + , K ( + ) - ATPase activity and that conditions that favored derepression do not allow for de novo synthesis of the Na + , K ( + ) - ATPase .
	manualset3
229127	6	421395	7	NULL	NULL	0	NULL	derepression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Indications are that the reduced Na + content in derepressed cells inhibits Na + , K ( + ) - ATPase activity and that conditions that favored derepression do not allow for de novo synthesis of the Na + , K ( + ) - ATPase .
	manualset3
229128	7	421395	7	NULL	NULL	0	NULL	 de novo synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Indications are that the reduced Na + content in derepressed cells inhibits Na + , K ( + ) - ATPase activity and that conditions that favored derepression do not allow for de novo synthesis of the Na + , K ( + ) - ATPase .
	manualset3
229129	8	421395	7	NULL	NULL	0	NULL	Na + , K ( + ) - ATPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Indications are that the reduced Na + content in derepressed cells inhibits Na + , K ( + ) - ATPase activity and that conditions that favored derepression do not allow for de novo synthesis of the Na + , K ( + ) - ATPase .
	manualset3
229130	1	421396	7	NULL	NULL	0	NULL	 authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors report about the course of pregnancy and delivery in two patients with cystic fibrosis .
	manualset3
229131	2	421396	7	NULL	NULL	0	NULL	course	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors report about the course of pregnancy and delivery in two patients with cystic fibrosis .
	manualset3
229132	3	421396	7	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors report about the course of pregnancy and delivery in two patients with cystic fibrosis .
	manualset3
229133	4	421396	7	NULL	NULL	0	NULL	delivery	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors report about the course of pregnancy and delivery in two patients with cystic fibrosis .
	manualset3
229134	5	421396	7	NULL	NULL	0	NULL	two patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors report about the course of pregnancy and delivery in two patients with cystic fibrosis .
	manualset3
229135	6	421396	7	NULL	NULL	0	NULL	cystic fibrosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors report about the course of pregnancy and delivery in two patients with cystic fibrosis .
	manualset3
229136	1	421397	7	NULL	NULL	0	NULL	Ab initio calculations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ab initio calculations are used to identify characteristics of vibrational and NMR spectra that signal the involvement of a protein backbone in a CH ... O H-bond and that distinguish this sort of interaction from other H-bonds in which a protein might participate .
	manualset3
229137	2	421397	7	NULL	NULL	0	NULL	characteristics	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ab initio calculations are used to identify characteristics of vibrational and NMR spectra that signal the involvement of a protein backbone in a CH ... O H-bond and that distinguish this sort of interaction from other H-bonds in which a protein might participate .
	manualset3
229138	3	421397	7	NULL	NULL	0	NULL	 vibrational spectra	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Ab initio calculations are used to identify characteristics of vibrational and NMR spectra that signal the involvement of a protein backbone in a CH ... O H-bond and that distinguish this sort of interaction from other H-bonds in which a protein might participate .
	manualset3
229139	4	421397	7	NULL	NULL	0	NULL	NMR spectra	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Ab initio calculations are used to identify characteristics of vibrational and NMR spectra that signal the involvement of a protein backbone in a CH ... O H-bond and that distinguish this sort of interaction from other H-bonds in which a protein might participate .
	manualset3
229140	5	421397	7	NULL	NULL	0	NULL	 involvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ab initio calculations are used to identify characteristics of vibrational and NMR spectra that signal the involvement of a protein backbone in a CH ... O H-bond and that distinguish this sort of interaction from other H-bonds in which a protein might participate .
	manualset3
229141	6	421397	7	NULL	NULL	0	NULL	protein backbone	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Ab initio calculations are used to identify characteristics of vibrational and NMR spectra that signal the involvement of a protein backbone in a CH ... O H-bond and that distinguish this sort of interaction from other H-bonds in which a protein might participate .
	manualset3
229142	7	421397	7	NULL	NULL	0	NULL	CH ... O H-bond	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ab initio calculations are used to identify characteristics of vibrational and NMR spectra that signal the involvement of a protein backbone in a CH ... O H-bond and that distinguish this sort of interaction from other H-bonds in which a protein might participate .
	manualset3
229143	8	421397	7	NULL	NULL	0	NULL	interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ab initio calculations are used to identify characteristics of vibrational and NMR spectra that signal the involvement of a protein backbone in a CH ... O H-bond and that distinguish this sort of interaction from other H-bonds in which a protein might participate .
	manualset3
229144	9	421397	7	NULL	NULL	0	NULL	H-bonds	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ab initio calculations are used to identify characteristics of vibrational and NMR spectra that signal the involvement of a protein backbone in a CH ... O H-bond and that distinguish this sort of interaction from other H-bonds in which a protein might participate .
	manualset3
229145	10	421397	7	NULL	NULL	0	NULL	protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Ab initio calculations are used to identify characteristics of vibrational and NMR spectra that signal the involvement of a protein backbone in a CH ... O H-bond and that distinguish this sort of interaction from other H-bonds in which a protein might participate .
	manualset3
229146	1	421398	7	NULL	NULL	0	NULL	FGA/89	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	FGA/89 and BR/90 were assayed for their neurovirulence in newborn mice , and neurons were the major target cells for both DEN-1 virus strains within the central nervous system .
	manualset3
229147	2	421398	7	NULL	NULL	0	NULL	BR/90	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	FGA/89 and BR/90 were assayed for their neurovirulence in newborn mice , and neurons were the major target cells for both DEN-1 virus strains within the central nervous system .
	manualset3
229148	3	421398	7	NULL	NULL	0	NULL	neurovirulence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	FGA/89 and BR/90 were assayed for their neurovirulence in newborn mice , and neurons were the major target cells for both DEN-1 virus strains within the central nervous system .
	manualset3
229149	4	421398	7	NULL	NULL	0	NULL	newborn mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	FGA/89 and BR/90 were assayed for their neurovirulence in newborn mice , and neurons were the major target cells for both DEN-1 virus strains within the central nervous system .
	manualset3
229150	5	421398	7	NULL	NULL	0	NULL	neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	FGA/89 and BR/90 were assayed for their neurovirulence in newborn mice , and neurons were the major target cells for both DEN-1 virus strains within the central nervous system .
	manualset3
229151	6	421398	7	NULL	NULL	0	NULL	major target cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	FGA/89 and BR/90 were assayed for their neurovirulence in newborn mice , and neurons were the major target cells for both DEN-1 virus strains within the central nervous system .
	manualset3
229152	7	421398	7	NULL	NULL	0	NULL	DEN-1 virus strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	FGA/89 and BR/90 were assayed for their neurovirulence in newborn mice , and neurons were the major target cells for both DEN-1 virus strains within the central nervous system .
	manualset3
229153	8	421398	7	NULL	NULL	0	NULL	central nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	FGA/89 and BR/90 were assayed for their neurovirulence in newborn mice , and neurons were the major target cells for both DEN-1 virus strains within the central nervous system .
	manualset3
229154	1	421399	7	NULL	NULL	0	NULL	No patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	No patient required more than 10 watt-seconds of energy for defibrillation , and , in 21 of them , 5 watt-seconds or less were sufficient .
	manualset3
229155	2	421399	7	NULL	NULL	0	NULL	10 watt-seconds	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	No patient required more than 10 watt-seconds of energy for defibrillation , and , in 21 of them , 5 watt-seconds or less were sufficient .
	manualset3
229156	3	421399	7	NULL	NULL	0	NULL	energy	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	No patient required more than 10 watt-seconds of energy for defibrillation , and , in 21 of them , 5 watt-seconds or less were sufficient .
	manualset3
229157	4	421399	7	NULL	NULL	0	NULL	defibrillation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	No patient required more than 10 watt-seconds of energy for defibrillation , and , in 21 of them , 5 watt-seconds or less were sufficient .
	manualset3
229158	5	421399	7	NULL	NULL	0	NULL	21	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	No patient required more than 10 watt-seconds of energy for defibrillation , and , in 21 of them , 5 watt-seconds or less were sufficient .
	manualset3
229159	6	421399	7	NULL	NULL	0	NULL	 5 watt-seconds	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	No patient required more than 10 watt-seconds of energy for defibrillation , and , in 21 of them , 5 watt-seconds or less were sufficient .
	manualset3
229160	1	421400	7	NULL	NULL	0	NULL	observed boost 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The observed boost in wt and rAAV production by HPV genes was not unexpected , as the Ad and HPV helper gene sets do not seem to recapitulate each other .
	manualset3
229161	2	421400	7	NULL	NULL	0	NULL	wt	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The observed boost in wt and rAAV production by HPV genes was not unexpected , as the Ad and HPV helper gene sets do not seem to recapitulate each other .
	manualset3
229162	3	421400	7	NULL	NULL	0	NULL	 rAAV production 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The observed boost in wt and rAAV production by HPV genes was not unexpected , as the Ad and HPV helper gene sets do not seem to recapitulate each other .
	manualset3
229163	4	421400	7	NULL	NULL	0	NULL	HPV genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The observed boost in wt and rAAV production by HPV genes was not unexpected , as the Ad and HPV helper gene sets do not seem to recapitulate each other .
	manualset3
229164	5	421400	7	NULL	NULL	0	NULL	Ad gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The observed boost in wt and rAAV production by HPV genes was not unexpected , as the Ad and HPV helper gene sets do not seem to recapitulate each other .
	manualset3
229165	6	421400	7	NULL	NULL	0	NULL	HPV helper gene sets	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The observed boost in wt and rAAV production by HPV genes was not unexpected , as the Ad and HPV helper gene sets do not seem to recapitulate each other .
	manualset3
229166	1	421401	7	NULL	NULL	0	NULL	extrahepatic manifestations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The extrahepatic manifestations of hepatocellular carcinoma are not uncommon , but have received little attention in the radiologic literature .
	manualset3
229167	2	421401	7	NULL	NULL	0	NULL	hepatocellular carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The extrahepatic manifestations of hepatocellular carcinoma are not uncommon , but have received little attention in the radiologic literature .
	manualset3
229168	3	421401	7	NULL	NULL	0	NULL	 little attention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The extrahepatic manifestations of hepatocellular carcinoma are not uncommon , but have received little attention in the radiologic literature .
	manualset3
229169	4	421401	7	NULL	NULL	0	NULL	radiologic literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The extrahepatic manifestations of hepatocellular carcinoma are not uncommon , but have received little attention in the radiologic literature .
	manualset3
229170	1	421402	7	NULL	NULL	0	NULL	accurate soft tissue substitution	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An accurate soft tissue substitution with creation of multiple subcutaneous and intramuscular tunnels for lipografting ensured adequate blood supply of the transplanted fat .
	manualset3
229171	2	421402	7	NULL	NULL	0	NULL	creation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An accurate soft tissue substitution with creation of multiple subcutaneous and intramuscular tunnels for lipografting ensured adequate blood supply of the transplanted fat .
	manualset3
229172	3	421402	7	NULL	NULL	0	NULL	multiple subcutaneous tunnels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An accurate soft tissue substitution with creation of multiple subcutaneous and intramuscular tunnels for lipografting ensured adequate blood supply of the transplanted fat .
	manualset3
229173	4	421402	7	NULL	NULL	0	NULL	intramuscular tunnels 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An accurate soft tissue substitution with creation of multiple subcutaneous and intramuscular tunnels for lipografting ensured adequate blood supply of the transplanted fat .
	manualset3
229174	5	421402	7	NULL	NULL	0	NULL	lipografting	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An accurate soft tissue substitution with creation of multiple subcutaneous and intramuscular tunnels for lipografting ensured adequate blood supply of the transplanted fat .
	manualset3
229175	6	421402	7	NULL	NULL	0	NULL	blood supply	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An accurate soft tissue substitution with creation of multiple subcutaneous and intramuscular tunnels for lipografting ensured adequate blood supply of the transplanted fat .
	manualset3
229176	7	421402	7	NULL	NULL	0	NULL	transplanted fat	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An accurate soft tissue substitution with creation of multiple subcutaneous and intramuscular tunnels for lipografting ensured adequate blood supply of the transplanted fat .
	manualset3
229177	1	421403	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the average velocity and standard deviation of velocity increased in the WL group but this was only statistically significant when the eyes were open .
	manualset3
229178	2	421403	7	NULL	NULL	0	NULL	average velocity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the average velocity and standard deviation of velocity increased in the WL group but this was only statistically significant when the eyes were open .
	manualset3
229179	3	421403	7	NULL	NULL	0	NULL	standard deviation	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the average velocity and standard deviation of velocity increased in the WL group but this was only statistically significant when the eyes were open .
	manualset3
229180	4	421403	7	NULL	NULL	0	NULL	velocity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the average velocity and standard deviation of velocity increased in the WL group but this was only statistically significant when the eyes were open .
	manualset3
229181	5	421403	7	NULL	NULL	0	NULL	WL group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the average velocity and standard deviation of velocity increased in the WL group but this was only statistically significant when the eyes were open .
	manualset3
229182	6	421403	7	NULL	NULL	0	NULL	eyes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the average velocity and standard deviation of velocity increased in the WL group but this was only statistically significant when the eyes were open .
	manualset3
229183	1	421404	7	NULL	NULL	0	NULL	 review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The following review contains three parts focusing respectively on basic knowledge of neuronal death and redox regulation , the mechanisms involved in neuronal death which are ordered in three sequential phases , and on the complex relations between neuronal fate and the redox status .
	manualset3
229184	2	421404	7	NULL	NULL	0	NULL	three parts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The following review contains three parts focusing respectively on basic knowledge of neuronal death and redox regulation , the mechanisms involved in neuronal death which are ordered in three sequential phases , and on the complex relations between neuronal fate and the redox status .
	manualset3
229185	3	421404	7	NULL	NULL	0	NULL	 basic knowledge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The following review contains three parts focusing respectively on basic knowledge of neuronal death and redox regulation , the mechanisms involved in neuronal death which are ordered in three sequential phases , and on the complex relations between neuronal fate and the redox status .
	manualset3
229186	4	421404	7	NULL	NULL	0	NULL	neuronal death 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The following review contains three parts focusing respectively on basic knowledge of neuronal death and redox regulation , the mechanisms involved in neuronal death which are ordered in three sequential phases , and on the complex relations between neuronal fate and the redox status .
	manualset3
229187	5	421404	7	NULL	NULL	0	NULL	redox regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The following review contains three parts focusing respectively on basic knowledge of neuronal death and redox regulation , the mechanisms involved in neuronal death which are ordered in three sequential phases , and on the complex relations between neuronal fate and the redox status .
	manualset3
229188	6	421404	7	NULL	NULL	0	NULL	mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The following review contains three parts focusing respectively on basic knowledge of neuronal death and redox regulation , the mechanisms involved in neuronal death which are ordered in three sequential phases , and on the complex relations between neuronal fate and the redox status .
	manualset3
229189	7	421404	7	NULL	NULL	0	NULL	neuronal death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The following review contains three parts focusing respectively on basic knowledge of neuronal death and redox regulation , the mechanisms involved in neuronal death which are ordered in three sequential phases , and on the complex relations between neuronal fate and the redox status .
	manualset3
229190	8	421404	7	NULL	NULL	0	NULL	three sequential phases	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The following review contains three parts focusing respectively on basic knowledge of neuronal death and redox regulation , the mechanisms involved in neuronal death which are ordered in three sequential phases , and on the complex relations between neuronal fate and the redox status .
	manualset3
229191	9	421404	7	NULL	NULL	0	NULL	complex relations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The following review contains three parts focusing respectively on basic knowledge of neuronal death and redox regulation , the mechanisms involved in neuronal death which are ordered in three sequential phases , and on the complex relations between neuronal fate and the redox status .
	manualset3
229192	10	421404	7	NULL	NULL	0	NULL	neuronal fate 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The following review contains three parts focusing respectively on basic knowledge of neuronal death and redox regulation , the mechanisms involved in neuronal death which are ordered in three sequential phases , and on the complex relations between neuronal fate and the redox status .
	manualset3
229193	11	421404	7	NULL	NULL	0	NULL	redox status	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The following review contains three parts focusing respectively on basic knowledge of neuronal death and redox regulation , the mechanisms involved in neuronal death which are ordered in three sequential phases , and on the complex relations between neuronal fate and the redox status .
	manualset3
229194	1	421405	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Elucidating the relationship between insulin resistance associated with aging in females , and the cross-talk between estradiol , insulin , and insulin-like growth factor ( IGF-1 ) signaling pathways , will lead to a more complete understanding of the mechanism underlying estradiol-mediated neuroprotection .
	manualset3
229195	2	421405	7	NULL	NULL	0	NULL	insulin resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Elucidating the relationship between insulin resistance associated with aging in females , and the cross-talk between estradiol , insulin , and insulin-like growth factor ( IGF-1 ) signaling pathways , will lead to a more complete understanding of the mechanism underlying estradiol-mediated neuroprotection .
	manualset3
229196	3	421405	7	NULL	NULL	0	NULL	aging	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Elucidating the relationship between insulin resistance associated with aging in females , and the cross-talk between estradiol , insulin , and insulin-like growth factor ( IGF-1 ) signaling pathways , will lead to a more complete understanding of the mechanism underlying estradiol-mediated neuroprotection .
	manualset3
229197	4	421405	7	NULL	NULL	0	NULL	females	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Elucidating the relationship between insulin resistance associated with aging in females , and the cross-talk between estradiol , insulin , and insulin-like growth factor ( IGF-1 ) signaling pathways , will lead to a more complete understanding of the mechanism underlying estradiol-mediated neuroprotection .
	manualset3
229198	5	421405	7	NULL	NULL	0	NULL	cross-talk	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Elucidating the relationship between insulin resistance associated with aging in females , and the cross-talk between estradiol , insulin , and insulin-like growth factor ( IGF-1 ) signaling pathways , will lead to a more complete understanding of the mechanism underlying estradiol-mediated neuroprotection .
	manualset3
229199	6	421405	7	NULL	NULL	0	NULL	estradiol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Elucidating the relationship between insulin resistance associated with aging in females , and the cross-talk between estradiol , insulin , and insulin-like growth factor ( IGF-1 ) signaling pathways , will lead to a more complete understanding of the mechanism underlying estradiol-mediated neuroprotection .
	manualset3
229200	7	421405	7	NULL	NULL	0	NULL	insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Elucidating the relationship between insulin resistance associated with aging in females , and the cross-talk between estradiol , insulin , and insulin-like growth factor ( IGF-1 ) signaling pathways , will lead to a more complete understanding of the mechanism underlying estradiol-mediated neuroprotection .
	manualset3
229201	8	421405	7	NULL	NULL	0	NULL	insulin-like growth factor ( IGF-1 ) signaling pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Elucidating the relationship between insulin resistance associated with aging in females , and the cross-talk between estradiol , insulin , and insulin-like growth factor ( IGF-1 ) signaling pathways , will lead to a more complete understanding of the mechanism underlying estradiol-mediated neuroprotection .
	manualset3
229202	9	421405	7	NULL	NULL	0	NULL	complete understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Elucidating the relationship between insulin resistance associated with aging in females , and the cross-talk between estradiol , insulin , and insulin-like growth factor ( IGF-1 ) signaling pathways , will lead to a more complete understanding of the mechanism underlying estradiol-mediated neuroprotection .
	manualset3
229203	10	421405	7	NULL	NULL	0	NULL	mechanism 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Elucidating the relationship between insulin resistance associated with aging in females , and the cross-talk between estradiol , insulin , and insulin-like growth factor ( IGF-1 ) signaling pathways , will lead to a more complete understanding of the mechanism underlying estradiol-mediated neuroprotection .
	manualset3
229204	11	421405	7	NULL	NULL	NULL	NULL	estradiol-mediated neuroprotection	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Elucidating the relationship between insulin resistance associated with aging in females , and the cross-talk between estradiol , insulin , and insulin-like growth factor ( IGF-1 ) signaling pathways , will lead to a more complete understanding of the mechanism underlying estradiol-mediated neuroprotection .
	manualset3
229205	1	421406	7	NULL	NULL	0	NULL	41 testicular germ cell tumors ( TGCT )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 41 testicular germ cell tumors ( TGCT ) using DNA flow cytometry and argyrophilic ( silver staining ) nucleolar organizer region ( Ag-NOR ) quantitation to evaluate the proliferative characteristics of TGCT and the significance of those analytical techniques .
	manualset3
229206	2	421406	7	NULL	NULL	0	NULL	DNA flow cytometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 41 testicular germ cell tumors ( TGCT ) using DNA flow cytometry and argyrophilic ( silver staining ) nucleolar organizer region ( Ag-NOR ) quantitation to evaluate the proliferative characteristics of TGCT and the significance of those analytical techniques .
	manualset3
229207	3	421406	7	NULL	NULL	0	NULL	argyrophilic ( silver staining ) nucleolar organizer region ( Ag-NOR ) quantitation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 41 testicular germ cell tumors ( TGCT ) using DNA flow cytometry and argyrophilic ( silver staining ) nucleolar organizer region ( Ag-NOR ) quantitation to evaluate the proliferative characteristics of TGCT and the significance of those analytical techniques .
	manualset3
229208	4	421406	7	NULL	NULL	0	NULL	proliferative characteristics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 41 testicular germ cell tumors ( TGCT ) using DNA flow cytometry and argyrophilic ( silver staining ) nucleolar organizer region ( Ag-NOR ) quantitation to evaluate the proliferative characteristics of TGCT and the significance of those analytical techniques .
	manualset3
229209	5	421406	7	NULL	NULL	0	NULL	TGCT	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 41 testicular germ cell tumors ( TGCT ) using DNA flow cytometry and argyrophilic ( silver staining ) nucleolar organizer region ( Ag-NOR ) quantitation to evaluate the proliferative characteristics of TGCT and the significance of those analytical techniques .
	manualset3
229210	6	421406	7	NULL	NULL	0	NULL	significance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 41 testicular germ cell tumors ( TGCT ) using DNA flow cytometry and argyrophilic ( silver staining ) nucleolar organizer region ( Ag-NOR ) quantitation to evaluate the proliferative characteristics of TGCT and the significance of those analytical techniques .
	manualset3
229211	7	421406	7	NULL	NULL	0	NULL	analytical techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied 41 testicular germ cell tumors ( TGCT ) using DNA flow cytometry and argyrophilic ( silver staining ) nucleolar organizer region ( Ag-NOR ) quantitation to evaluate the proliferative characteristics of TGCT and the significance of those analytical techniques .
	manualset3
229212	1	421407	7	NULL	NULL	0	NULL	Region IV	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Region IV contained an even more polar material , probably including conjugates of HCB metabolites .
	manualset3
229213	2	421407	7	NULL	NULL	0	NULL	 polar material	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Region IV contained an even more polar material , probably including conjugates of HCB metabolites .
	manualset3
229214	3	421407	7	NULL	NULL	0	NULL	conjugates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Region IV contained an even more polar material , probably including conjugates of HCB metabolites .
	manualset3
229215	4	421407	7	NULL	NULL	0	NULL	HCB metabolites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Region IV contained an even more polar material , probably including conjugates of HCB metabolites .
	manualset3
229216	1	421408	7	NULL	NULL	0	NULL	 rate of change	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of change for temporal lobe areas remained constant over different AD stages , whereas those for corpus callosum width and for cognitive impairment were greater for severe cases ( p & lt ; 0.05 ) .
	manualset3
229217	2	421408	7	NULL	NULL	0	NULL	temporal lobe areas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of change for temporal lobe areas remained constant over different AD stages , whereas those for corpus callosum width and for cognitive impairment were greater for severe cases ( p & lt ; 0.05 ) .
	manualset3
229218	3	421408	7	NULL	NULL	0	NULL	different AD stages	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of change for temporal lobe areas remained constant over different AD stages , whereas those for corpus callosum width and for cognitive impairment were greater for severe cases ( p & lt ; 0.05 ) .
	manualset3
229219	4	421408	7	NULL	NULL	NULL	NULL	corpus callosum width	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The rate of change for temporal lobe areas remained constant over different AD stages , whereas those for corpus callosum width and for cognitive impairment were greater for severe cases ( p & lt ; 0.05 ) .
	manualset3
229220	5	421408	7	NULL	NULL	0	NULL	cognitive impairment	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of change for temporal lobe areas remained constant over different AD stages , whereas those for corpus callosum width and for cognitive impairment were greater for severe cases ( p & lt ; 0.05 ) .
	manualset3
229221	6	421408	7	NULL	NULL	0	NULL	severe cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of change for temporal lobe areas remained constant over different AD stages , whereas those for corpus callosum width and for cognitive impairment were greater for severe cases ( p & lt ; 0.05 ) .
	manualset3
229222	7	421408	7	NULL	NULL	0	NULL	p & lt ; 0.05 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of change for temporal lobe areas remained constant over different AD stages , whereas those for corpus callosum width and for cognitive impairment were greater for severe cases ( p & lt ; 0.05 ) .
	manualset3
229223	1	421409	7	NULL	NULL	0	NULL	Proceedings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceedings of the National Academy of Sciences of the United States of America , August 1975 , Volume 72 : Thromboxanes : a new group of biologically active compounds derived from prostaglandin endoperoxides .
	manualset3
229224	2	421409	7	NULL	NULL	0	NULL	National Academy of Sciences	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceedings of the National Academy of Sciences of the United States of America , August 1975 , Volume 72 : Thromboxanes : a new group of biologically active compounds derived from prostaglandin endoperoxides .
	manualset3
229225	3	421409	7	NULL	NULL	0	NULL	United States of America	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceedings of the National Academy of Sciences of the United States of America , August 1975 , Volume 72 : Thromboxanes : a new group of biologically active compounds derived from prostaglandin endoperoxides .
	manualset3
229226	4	421409	7	NULL	NULL	0	NULL	August 1975 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceedings of the National Academy of Sciences of the United States of America , August 1975 , Volume 72 : Thromboxanes : a new group of biologically active compounds derived from prostaglandin endoperoxides .
	manualset3
229227	5	421409	7	NULL	NULL	0	NULL	Volume 72	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceedings of the National Academy of Sciences of the United States of America , August 1975 , Volume 72 : Thromboxanes : a new group of biologically active compounds derived from prostaglandin endoperoxides .
	manualset3
229228	6	421409	7	NULL	NULL	0	NULL	Thromboxanes	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceedings of the National Academy of Sciences of the United States of America , August 1975 , Volume 72 : Thromboxanes : a new group of biologically active compounds derived from prostaglandin endoperoxides .
	manualset3
229229	7	421409	7	NULL	NULL	0	NULL	new group	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceedings of the National Academy of Sciences of the United States of America , August 1975 , Volume 72 : Thromboxanes : a new group of biologically active compounds derived from prostaglandin endoperoxides .
	manualset3
229230	8	421409	7	NULL	NULL	0	NULL	biologically active compounds	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceedings of the National Academy of Sciences of the United States of America , August 1975 , Volume 72 : Thromboxanes : a new group of biologically active compounds derived from prostaglandin endoperoxides .
	manualset3
229231	9	421409	7	NULL	NULL	0	NULL	prostaglandin endoperoxides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Proceedings of the National Academy of Sciences of the United States of America , August 1975 , Volume 72 : Thromboxanes : a new group of biologically active compounds derived from prostaglandin endoperoxides .
	manualset3
229232	1	421410	7	NULL	NULL	0	NULL	experiment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This experiment suggests one of the defense mechanisms of the vesical epithelium againts E. coli .
	manualset3
229233	2	421410	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This experiment suggests one of the defense mechanisms of the vesical epithelium againts E. coli .
	manualset3
229234	3	421410	7	NULL	NULL	0	NULL	defense mechanisms 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This experiment suggests one of the defense mechanisms of the vesical epithelium againts E. coli .
	manualset3
229235	4	421410	7	NULL	NULL	0	NULL	vesical epithelium	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	This experiment suggests one of the defense mechanisms of the vesical epithelium againts E. coli .
	manualset3
229236	5	421410	7	NULL	NULL	0	NULL	 E. coli 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	This experiment suggests one of the defense mechanisms of the vesical epithelium againts E. coli .
	manualset3
229237	1	421411	7	NULL	NULL	0	NULL	Members	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of the genera Aurantimonas and Fulvimarina have largely been described on the basis of 16S rRNA gene sequence analyses , biochemical tests and limited chemotaxonomic data .
	manualset3
229238	2	421411	7	NULL	NULL	0	NULL	genera Aurantimonas 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of the genera Aurantimonas and Fulvimarina have largely been described on the basis of 16S rRNA gene sequence analyses , biochemical tests and limited chemotaxonomic data .
	manualset3
229239	3	421411	7	NULL	NULL	0	NULL	Fulvimarina 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of the genera Aurantimonas and Fulvimarina have largely been described on the basis of 16S rRNA gene sequence analyses , biochemical tests and limited chemotaxonomic data .
	manualset3
229240	4	421411	7	NULL	NULL	0	NULL	basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of the genera Aurantimonas and Fulvimarina have largely been described on the basis of 16S rRNA gene sequence analyses , biochemical tests and limited chemotaxonomic data .
	manualset3
229241	5	421411	7	NULL	NULL	0	NULL	16S rRNA gene sequence analyses	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of the genera Aurantimonas and Fulvimarina have largely been described on the basis of 16S rRNA gene sequence analyses , biochemical tests and limited chemotaxonomic data .
	manualset3
229242	6	421411	7	NULL	NULL	0	NULL	biochemical tests	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of the genera Aurantimonas and Fulvimarina have largely been described on the basis of 16S rRNA gene sequence analyses , biochemical tests and limited chemotaxonomic data .
	manualset3
229243	7	421411	7	NULL	NULL	0	NULL	chemotaxonomic data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Members of the genera Aurantimonas and Fulvimarina have largely been described on the basis of 16S rRNA gene sequence analyses , biochemical tests and limited chemotaxonomic data .
	manualset3
229244	1	421412	7	NULL	NULL	0	NULL	environmental factors	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	An acquired and environmental factors were assumed to be involved in this disease because the correlation between allelic frequencies and coronary artery disease status showed dilution when the subject age distribution included older subjects .
	manualset3
229245	2	421412	7	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	An acquired and environmental factors were assumed to be involved in this disease because the correlation between allelic frequencies and coronary artery disease status showed dilution when the subject age distribution included older subjects .
	manualset3
229246	3	421412	7	NULL	NULL	0	NULL	 correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	An acquired and environmental factors were assumed to be involved in this disease because the correlation between allelic frequencies and coronary artery disease status showed dilution when the subject age distribution included older subjects .
	manualset3
229247	4	421412	7	NULL	NULL	0	NULL	allelic frequencies	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An acquired and environmental factors were assumed to be involved in this disease because the correlation between allelic frequencies and coronary artery disease status showed dilution when the subject age distribution included older subjects .
	manualset3
229248	5	421412	7	NULL	NULL	0	NULL	coronary artery disease status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An acquired and environmental factors were assumed to be involved in this disease because the correlation between allelic frequencies and coronary artery disease status showed dilution when the subject age distribution included older subjects .
	manualset3
229249	6	421412	7	NULL	NULL	0	NULL	dilution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An acquired and environmental factors were assumed to be involved in this disease because the correlation between allelic frequencies and coronary artery disease status showed dilution when the subject age distribution included older subjects .
	manualset3
229250	7	421412	7	NULL	NULL	NULL	NULL	subject 	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An acquired and environmental factors were assumed to be involved in this disease because the correlation between allelic frequencies and coronary artery disease status showed dilution when the subject age distribution included older subjects .
	manualset3
229251	8	421412	7	NULL	NULL	0	NULL	older subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	An acquired and environmental factors were assumed to be involved in this disease because the correlation between allelic frequencies and coronary artery disease status showed dilution when the subject age distribution included older subjects .
	manualset3
230552	9	421412	7	NULL	NULL	NULL	NULL	subject age distribution	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An acquired and environmental factors were assumed to be involved in this disease because the correlation between allelic frequencies and coronary artery disease status showed dilution when the subject age distribution included older subjects .
	manualset3
229252	1	421413	7	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss recent advances in our understanding of the Ndc80 complex and address future areas of research .
	manualset3
229253	2	421413	7	NULL	NULL	0	NULL	recent advances	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss recent advances in our understanding of the Ndc80 complex and address future areas of research .
	manualset3
229254	3	421413	7	NULL	NULL	0	NULL	understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss recent advances in our understanding of the Ndc80 complex and address future areas of research .
	manualset3
229255	4	421413	7	NULL	NULL	0	NULL	Ndc80 complex 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss recent advances in our understanding of the Ndc80 complex and address future areas of research .
	manualset3
229256	5	421413	7	NULL	NULL	NULL	NULL	future areas	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this review , we discuss recent advances in our understanding of the Ndc80 complex and address future areas of research .
	manualset3
229257	6	421413	7	NULL	NULL	0	NULL	research 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this review , we discuss recent advances in our understanding of the Ndc80 complex and address future areas of research .
	manualset3
229258	1	421414	7	NULL	NULL	0	NULL	Objective evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective and functional evaluation was performed after median 37 ( range 24-87 ) months by two independent observers using the International Knee Documentation Committee ( IKDC ) knee evaluation form , the Lysholm knee function score , and the Tegner activity score .
	manualset3
229259	2	421414	7	NULL	NULL	0	NULL	functional evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective and functional evaluation was performed after median 37 ( range 24-87 ) months by two independent observers using the International Knee Documentation Committee ( IKDC ) knee evaluation form , the Lysholm knee function score , and the Tegner activity score .
	manualset3
229260	3	421414	7	NULL	NULL	NULL	NULL	median 37 months	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Objective and functional evaluation was performed after median 37 ( range 24-87 ) months by two independent observers using the International Knee Documentation Committee ( IKDC ) knee evaluation form , the Lysholm knee function score , and the Tegner activity score .
	manualset3
229261	4	421414	7	NULL	NULL	0	NULL	range 24-87	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective and functional evaluation was performed after median 37 ( range 24-87 ) months by two independent observers using the International Knee Documentation Committee ( IKDC ) knee evaluation form , the Lysholm knee function score , and the Tegner activity score .
	manualset3
229262	5	421414	7	NULL	NULL	0	NULL	two independent observers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective and functional evaluation was performed after median 37 ( range 24-87 ) months by two independent observers using the International Knee Documentation Committee ( IKDC ) knee evaluation form , the Lysholm knee function score , and the Tegner activity score .
	manualset3
229263	6	421414	7	NULL	NULL	0	NULL	International Knee Documentation Committee ( IKDC ) 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective and functional evaluation was performed after median 37 ( range 24-87 ) months by two independent observers using the International Knee Documentation Committee ( IKDC ) knee evaluation form , the Lysholm knee function score , and the Tegner activity score .
	manualset3
229264	7	421414	7	NULL	NULL	0	NULL	knee evaluation form	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective and functional evaluation was performed after median 37 ( range 24-87 ) months by two independent observers using the International Knee Documentation Committee ( IKDC ) knee evaluation form , the Lysholm knee function score , and the Tegner activity score .
	manualset3
229265	8	421414	7	NULL	NULL	0	NULL	Lysholm knee function score 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective and functional evaluation was performed after median 37 ( range 24-87 ) months by two independent observers using the International Knee Documentation Committee ( IKDC ) knee evaluation form , the Lysholm knee function score , and the Tegner activity score .
	manualset3
229266	9	421414	7	NULL	NULL	0	NULL	Tegner activity score	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Objective and functional evaluation was performed after median 37 ( range 24-87 ) months by two independent observers using the International Knee Documentation Committee ( IKDC ) knee evaluation form , the Lysholm knee function score , and the Tegner activity score .
	manualset3
229267	1	421415	7	NULL	NULL	0	NULL	Salicylates 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Salicylates were believed to be well tolerated , but recent reports have demonstrated that diflunisal and salicylsalicylic acid can precipitate asthma attacks in aspirin-intolerant patients .
	manualset3
229268	2	421415	7	NULL	NULL	0	NULL	recent reports	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Salicylates were believed to be well tolerated , but recent reports have demonstrated that diflunisal and salicylsalicylic acid can precipitate asthma attacks in aspirin-intolerant patients .
	manualset3
229269	3	421415	7	NULL	NULL	0	NULL	diflunisal	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Salicylates were believed to be well tolerated , but recent reports have demonstrated that diflunisal and salicylsalicylic acid can precipitate asthma attacks in aspirin-intolerant patients .
	manualset3
229270	4	421415	7	NULL	NULL	0	NULL	salicylsalicylic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Salicylates were believed to be well tolerated , but recent reports have demonstrated that diflunisal and salicylsalicylic acid can precipitate asthma attacks in aspirin-intolerant patients .
	manualset3
229271	5	421415	7	NULL	NULL	0	NULL	asthma attacks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Salicylates were believed to be well tolerated , but recent reports have demonstrated that diflunisal and salicylsalicylic acid can precipitate asthma attacks in aspirin-intolerant patients .
	manualset3
229272	6	421415	7	NULL	NULL	0	NULL	aspirin-intolerant patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Salicylates were believed to be well tolerated , but recent reports have demonstrated that diflunisal and salicylsalicylic acid can precipitate asthma attacks in aspirin-intolerant patients .
	manualset3
229273	1	421416	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results implicate the calcium-calmodulin pathway in the mechanisms for regulating MAPK activity and the resultant c-fos expression induced by BK in VSMC .
	manualset3
229274	2	421416	7	NULL	NULL	0	NULL	calcium-calmodulin pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results implicate the calcium-calmodulin pathway in the mechanisms for regulating MAPK activity and the resultant c-fos expression induced by BK in VSMC .
	manualset3
229275	3	421416	7	NULL	NULL	0	NULL	mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results implicate the calcium-calmodulin pathway in the mechanisms for regulating MAPK activity and the resultant c-fos expression induced by BK in VSMC .
	manualset3
229276	4	421416	7	NULL	NULL	0	NULL	MAPK activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results implicate the calcium-calmodulin pathway in the mechanisms for regulating MAPK activity and the resultant c-fos expression induced by BK in VSMC .
	manualset3
229277	5	421416	7	NULL	NULL	0	NULL	c-fos expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results implicate the calcium-calmodulin pathway in the mechanisms for regulating MAPK activity and the resultant c-fos expression induced by BK in VSMC .
	manualset3
229278	6	421416	7	NULL	NULL	0	NULL	BK	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	These results implicate the calcium-calmodulin pathway in the mechanisms for regulating MAPK activity and the resultant c-fos expression induced by BK in VSMC .
	manualset3
229279	7	421416	7	NULL	NULL	0	NULL	VSMC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These results implicate the calcium-calmodulin pathway in the mechanisms for regulating MAPK activity and the resultant c-fos expression induced by BK in VSMC .
	manualset3
229280	1	421417	7	NULL	NULL	0	NULL	new method 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A new method of introducing sulfonic acid or nitrile groups into position 4 of the pyridine nucleus ) .
	manualset3
229281	2	421417	7	NULL	NULL	0	NULL	sulfonic acid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A new method of introducing sulfonic acid or nitrile groups into position 4 of the pyridine nucleus ) .
	manualset3
229282	3	421417	7	NULL	NULL	0	NULL	 nitrile groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A new method of introducing sulfonic acid or nitrile groups into position 4 of the pyridine nucleus ) .
	manualset3
229283	4	421417	7	NULL	NULL	0	NULL	position 4	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A new method of introducing sulfonic acid or nitrile groups into position 4 of the pyridine nucleus ) .
	manualset3
229284	5	421417	7	NULL	NULL	0	NULL	pyridine nucleus	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A new method of introducing sulfonic acid or nitrile groups into position 4 of the pyridine nucleus ) .
	manualset3
229285	1	421418	7	NULL	NULL	0	NULL	Comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the reliability and validity of outcome instruments for cutaneous dermatomyositis .
	manualset3
229286	2	421418	7	NULL	NULL	0	NULL	reliability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the reliability and validity of outcome instruments for cutaneous dermatomyositis .
	manualset3
229287	3	421418	7	NULL	NULL	0	NULL	validity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the reliability and validity of outcome instruments for cutaneous dermatomyositis .
	manualset3
229288	4	421418	7	NULL	NULL	0	NULL	outcome instruments	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the reliability and validity of outcome instruments for cutaneous dermatomyositis .
	manualset3
229289	5	421418	7	NULL	NULL	0	NULL	cutaneous dermatomyositis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the reliability and validity of outcome instruments for cutaneous dermatomyositis .
	manualset3
229290	1	421419	7	NULL	NULL	0	NULL	introduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After the introduction of ionomycin in the medium , ( Ca2 + ) i increased gradually and reached a plateau in approximately 30 s. The fusion of the acrosomal vacuole took place abruptly before the plateau , during the rising phase .
	manualset3
229291	2	421419	7	NULL	NULL	0	NULL	ionomycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	After the introduction of ionomycin in the medium , ( Ca2 + ) i increased gradually and reached a plateau in approximately 30 s. The fusion of the acrosomal vacuole took place abruptly before the plateau , during the rising phase .
	manualset3
229292	3	421419	7	NULL	NULL	0	NULL	medium	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	After the introduction of ionomycin in the medium , ( Ca2 + ) i increased gradually and reached a plateau in approximately 30 s. The fusion of the acrosomal vacuole took place abruptly before the plateau , during the rising phase .
	manualset3
229293	4	421419	7	NULL	NULL	0	NULL	( Ca2 + ) i 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	After the introduction of ionomycin in the medium , ( Ca2 + ) i increased gradually and reached a plateau in approximately 30 s. The fusion of the acrosomal vacuole took place abruptly before the plateau , during the rising phase .
	manualset3
229294	5	421419	7	NULL	NULL	0	NULL	plateau	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After the introduction of ionomycin in the medium , ( Ca2 + ) i increased gradually and reached a plateau in approximately 30 s. The fusion of the acrosomal vacuole took place abruptly before the plateau , during the rising phase .
	manualset3
229295	6	421419	7	NULL	NULL	0	NULL	30 s	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	After the introduction of ionomycin in the medium , ( Ca2 + ) i increased gradually and reached a plateau in approximately 30 s. The fusion of the acrosomal vacuole took place abruptly before the plateau , during the rising phase .
	manualset3
229296	7	421419	7	NULL	NULL	0	NULL	fusion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	After the introduction of ionomycin in the medium , ( Ca2 + ) i increased gradually and reached a plateau in approximately 30 s. The fusion of the acrosomal vacuole took place abruptly before the plateau , during the rising phase .
	manualset3
229297	8	421419	7	NULL	NULL	0	NULL	acrosomal vacuole	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	After the introduction of ionomycin in the medium , ( Ca2 + ) i increased gradually and reached a plateau in approximately 30 s. The fusion of the acrosomal vacuole took place abruptly before the plateau , during the rising phase .
	manualset3
229298	9	421419	7	NULL	NULL	0	NULL	plateau	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After the introduction of ionomycin in the medium , ( Ca2 + ) i increased gradually and reached a plateau in approximately 30 s. The fusion of the acrosomal vacuole took place abruptly before the plateau , during the rising phase .
	manualset3
229299	10	421419	7	NULL	NULL	0	NULL	rising phase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	After the introduction of ionomycin in the medium , ( Ca2 + ) i increased gradually and reached a plateau in approximately 30 s. The fusion of the acrosomal vacuole took place abruptly before the plateau , during the rising phase .
	manualset3
229300	1	421420	7	NULL	NULL	0	NULL	Glycosaminoglycans	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycosaminoglycans , uptake of 35S-sulphate , collagen , uptake of 125I-albumin , and vascular histochemistry and morphology were analyzed in the thoracic aorta .
	manualset3
229301	2	421420	7	NULL	NULL	0	NULL	uptake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycosaminoglycans , uptake of 35S-sulphate , collagen , uptake of 125I-albumin , and vascular histochemistry and morphology were analyzed in the thoracic aorta .
	manualset3
229302	3	421420	7	NULL	NULL	0	NULL	35S-sulphate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycosaminoglycans , uptake of 35S-sulphate , collagen , uptake of 125I-albumin , and vascular histochemistry and morphology were analyzed in the thoracic aorta .
	manualset3
229303	4	421420	7	NULL	NULL	0	NULL	collagen 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycosaminoglycans , uptake of 35S-sulphate , collagen , uptake of 125I-albumin , and vascular histochemistry and morphology were analyzed in the thoracic aorta .
	manualset3
229304	5	421420	7	NULL	NULL	0	NULL	uptake 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycosaminoglycans , uptake of 35S-sulphate , collagen , uptake of 125I-albumin , and vascular histochemistry and morphology were analyzed in the thoracic aorta .
	manualset3
229305	6	421420	7	NULL	NULL	0	NULL	125I-albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycosaminoglycans , uptake of 35S-sulphate , collagen , uptake of 125I-albumin , and vascular histochemistry and morphology were analyzed in the thoracic aorta .
	manualset3
229306	7	421420	7	NULL	NULL	0	NULL	vascular histochemistry	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycosaminoglycans , uptake of 35S-sulphate , collagen , uptake of 125I-albumin , and vascular histochemistry and morphology were analyzed in the thoracic aorta .
	manualset3
229307	8	421420	7	NULL	NULL	0	NULL	morphology	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycosaminoglycans , uptake of 35S-sulphate , collagen , uptake of 125I-albumin , and vascular histochemistry and morphology were analyzed in the thoracic aorta .
	manualset3
229308	9	421420	7	NULL	NULL	0	NULL	thoracic aorta	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Glycosaminoglycans , uptake of 35S-sulphate , collagen , uptake of 125I-albumin , and vascular histochemistry and morphology were analyzed in the thoracic aorta .
	manualset3
229309	1	421421	7	NULL	NULL	0	NULL	behavioral effects 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The behavioral effects correlated with the lost of tyrosine hydroxylase-positive staining , since animals unilaterally and intranigrally injected with 0.25 nmol of CuSO4 together with 2 nmol of dicoumarol exhibited extensive loss of tyrosine hydroxylase-positive fiber density in the striatum ( P & lt ; 0.01 ) and cell loss in the substantia nigra ( P & lt ; 0.01 ) .
	manualset3
229310	2	421421	7	NULL	NULL	0	NULL	tyrosine hydroxylase-positive staining	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The behavioral effects correlated with the lost of tyrosine hydroxylase-positive staining , since animals unilaterally and intranigrally injected with 0.25 nmol of CuSO4 together with 2 nmol of dicoumarol exhibited extensive loss of tyrosine hydroxylase-positive fiber density in the striatum ( P & lt ; 0.01 ) and cell loss in the substantia nigra ( P & lt ; 0.01 ) .
	manualset3
229311	3	421421	7	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The behavioral effects correlated with the lost of tyrosine hydroxylase-positive staining , since animals unilaterally and intranigrally injected with 0.25 nmol of CuSO4 together with 2 nmol of dicoumarol exhibited extensive loss of tyrosine hydroxylase-positive fiber density in the striatum ( P & lt ; 0.01 ) and cell loss in the substantia nigra ( P & lt ; 0.01 ) .
	manualset3
229312	4	421421	7	NULL	NULL	0	NULL	 0.25 nmol	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The behavioral effects correlated with the lost of tyrosine hydroxylase-positive staining , since animals unilaterally and intranigrally injected with 0.25 nmol of CuSO4 together with 2 nmol of dicoumarol exhibited extensive loss of tyrosine hydroxylase-positive fiber density in the striatum ( P & lt ; 0.01 ) and cell loss in the substantia nigra ( P & lt ; 0.01 ) .
	manualset3
229313	5	421421	7	NULL	NULL	0	NULL	CuSO4	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The behavioral effects correlated with the lost of tyrosine hydroxylase-positive staining , since animals unilaterally and intranigrally injected with 0.25 nmol of CuSO4 together with 2 nmol of dicoumarol exhibited extensive loss of tyrosine hydroxylase-positive fiber density in the striatum ( P & lt ; 0.01 ) and cell loss in the substantia nigra ( P & lt ; 0.01 ) .
	manualset3
229314	6	421421	7	NULL	NULL	0	NULL	 2 nmol	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The behavioral effects correlated with the lost of tyrosine hydroxylase-positive staining , since animals unilaterally and intranigrally injected with 0.25 nmol of CuSO4 together with 2 nmol of dicoumarol exhibited extensive loss of tyrosine hydroxylase-positive fiber density in the striatum ( P & lt ; 0.01 ) and cell loss in the substantia nigra ( P & lt ; 0.01 ) .
	manualset3
229315	7	421421	7	NULL	NULL	0	NULL	dicoumarol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The behavioral effects correlated with the lost of tyrosine hydroxylase-positive staining , since animals unilaterally and intranigrally injected with 0.25 nmol of CuSO4 together with 2 nmol of dicoumarol exhibited extensive loss of tyrosine hydroxylase-positive fiber density in the striatum ( P & lt ; 0.01 ) and cell loss in the substantia nigra ( P & lt ; 0.01 ) .
	manualset3
229316	8	421421	7	NULL	NULL	0	NULL	extensive loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The behavioral effects correlated with the lost of tyrosine hydroxylase-positive staining , since animals unilaterally and intranigrally injected with 0.25 nmol of CuSO4 together with 2 nmol of dicoumarol exhibited extensive loss of tyrosine hydroxylase-positive fiber density in the striatum ( P & lt ; 0.01 ) and cell loss in the substantia nigra ( P & lt ; 0.01 ) .
	manualset3
229317	9	421421	7	NULL	NULL	0	NULL	tyrosine hydroxylase-positive fiber density 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The behavioral effects correlated with the lost of tyrosine hydroxylase-positive staining , since animals unilaterally and intranigrally injected with 0.25 nmol of CuSO4 together with 2 nmol of dicoumarol exhibited extensive loss of tyrosine hydroxylase-positive fiber density in the striatum ( P & lt ; 0.01 ) and cell loss in the substantia nigra ( P & lt ; 0.01 ) .
	manualset3
229318	10	421421	7	NULL	NULL	0	NULL	striatum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The behavioral effects correlated with the lost of tyrosine hydroxylase-positive staining , since animals unilaterally and intranigrally injected with 0.25 nmol of CuSO4 together with 2 nmol of dicoumarol exhibited extensive loss of tyrosine hydroxylase-positive fiber density in the striatum ( P & lt ; 0.01 ) and cell loss in the substantia nigra ( P & lt ; 0.01 ) .
	manualset3
229319	11	421421	7	NULL	NULL	0	NULL	P & lt ; 0.01 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The behavioral effects correlated with the lost of tyrosine hydroxylase-positive staining , since animals unilaterally and intranigrally injected with 0.25 nmol of CuSO4 together with 2 nmol of dicoumarol exhibited extensive loss of tyrosine hydroxylase-positive fiber density in the striatum ( P & lt ; 0.01 ) and cell loss in the substantia nigra ( P & lt ; 0.01 ) .
	manualset3
229320	12	421421	7	NULL	NULL	0	NULL	cell loss 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The behavioral effects correlated with the lost of tyrosine hydroxylase-positive staining , since animals unilaterally and intranigrally injected with 0.25 nmol of CuSO4 together with 2 nmol of dicoumarol exhibited extensive loss of tyrosine hydroxylase-positive fiber density in the striatum ( P & lt ; 0.01 ) and cell loss in the substantia nigra ( P & lt ; 0.01 ) .
	manualset3
229321	13	421421	7	NULL	NULL	0	NULL	substantia nigra	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The behavioral effects correlated with the lost of tyrosine hydroxylase-positive staining , since animals unilaterally and intranigrally injected with 0.25 nmol of CuSO4 together with 2 nmol of dicoumarol exhibited extensive loss of tyrosine hydroxylase-positive fiber density in the striatum ( P & lt ; 0.01 ) and cell loss in the substantia nigra ( P & lt ; 0.01 ) .
	manualset3
229322	14	421421	7	NULL	NULL	0	NULL	P & lt ; 0.01 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The behavioral effects correlated with the lost of tyrosine hydroxylase-positive staining , since animals unilaterally and intranigrally injected with 0.25 nmol of CuSO4 together with 2 nmol of dicoumarol exhibited extensive loss of tyrosine hydroxylase-positive fiber density in the striatum ( P & lt ; 0.01 ) and cell loss in the substantia nigra ( P & lt ; 0.01 ) .
	manualset3
229323	1	421422	7	NULL	NULL	0	NULL	elastic bonding strength	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Depending on the elastic bonding strength , the band structure separates long-living surface acoustic waves with frequencies in the complete band gap from bulk waves with band frequencies that propagate into the crystal leading to a fast decay .
	manualset3
229324	2	421422	7	NULL	NULL	0	NULL	band structure 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Depending on the elastic bonding strength , the band structure separates long-living surface acoustic waves with frequencies in the complete band gap from bulk waves with band frequencies that propagate into the crystal leading to a fast decay .
	manualset3
229325	3	421422	7	NULL	NULL	0	NULL	long-living surface acoustic waves	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Depending on the elastic bonding strength , the band structure separates long-living surface acoustic waves with frequencies in the complete band gap from bulk waves with band frequencies that propagate into the crystal leading to a fast decay .
	manualset3
229326	4	421422	7	NULL	NULL	0	NULL	 frequencies	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Depending on the elastic bonding strength , the band structure separates long-living surface acoustic waves with frequencies in the complete band gap from bulk waves with band frequencies that propagate into the crystal leading to a fast decay .
	manualset3
229327	5	421422	7	NULL	NULL	0	NULL	complete band gap	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Depending on the elastic bonding strength , the band structure separates long-living surface acoustic waves with frequencies in the complete band gap from bulk waves with band frequencies that propagate into the crystal leading to a fast decay .
	manualset3
229328	6	421422	7	NULL	NULL	0	NULL	bulk waves	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Depending on the elastic bonding strength , the band structure separates long-living surface acoustic waves with frequencies in the complete band gap from bulk waves with band frequencies that propagate into the crystal leading to a fast decay .
	manualset3
229329	7	421422	7	NULL	NULL	0	NULL	band frequencies 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Depending on the elastic bonding strength , the band structure separates long-living surface acoustic waves with frequencies in the complete band gap from bulk waves with band frequencies that propagate into the crystal leading to a fast decay .
	manualset3
229330	8	421422	7	NULL	NULL	0	NULL	 crystal	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Depending on the elastic bonding strength , the band structure separates long-living surface acoustic waves with frequencies in the complete band gap from bulk waves with band frequencies that propagate into the crystal leading to a fast decay .
	manualset3
229331	9	421422	7	NULL	NULL	0	NULL	fast decay	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Depending on the elastic bonding strength , the band structure separates long-living surface acoustic waves with frequencies in the complete band gap from bulk waves with band frequencies that propagate into the crystal leading to a fast decay .
	manualset3
229332	1	421423	7	NULL	NULL	0	NULL	Cursive epilepsy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Cursive epilepsy and gelastic epilepsy .
	manualset3
229333	2	421423	7	NULL	NULL	0	NULL	gelastic epilepsy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Cursive epilepsy and gelastic epilepsy .
	manualset3
229334	1	421424	7	NULL	NULL	0	NULL	cytosolic concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ) The cytosolic concentration of G-actin is significantly reduced by an elevation in intravascular pressure , demonstrating the dynamic nature of actin within VSM and implying a shift in the F : G equilibrium in favor of F-actin .
	manualset3
229335	2	421424	7	NULL	NULL	0	NULL	G-actin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ) The cytosolic concentration of G-actin is significantly reduced by an elevation in intravascular pressure , demonstrating the dynamic nature of actin within VSM and implying a shift in the F : G equilibrium in favor of F-actin .
	manualset3
229336	3	421424	7	NULL	NULL	NULL	NULL	elevation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	2 ) The cytosolic concentration of G-actin is significantly reduced by an elevation in intravascular pressure , demonstrating the dynamic nature of actin within VSM and implying a shift in the F : G equilibrium in favor of F-actin .
	manualset3
229337	4	421424	7	NULL	NULL	0	NULL	intravascular pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ) The cytosolic concentration of G-actin is significantly reduced by an elevation in intravascular pressure , demonstrating the dynamic nature of actin within VSM and implying a shift in the F : G equilibrium in favor of F-actin .
	manualset3
229338	5	421424	7	NULL	NULL	NULL	NULL	 dynamic nature	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	2 ) The cytosolic concentration of G-actin is significantly reduced by an elevation in intravascular pressure , demonstrating the dynamic nature of actin within VSM and implying a shift in the F : G equilibrium in favor of F-actin .
	manualset3
229339	6	421424	7	NULL	NULL	0	NULL	actin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ) The cytosolic concentration of G-actin is significantly reduced by an elevation in intravascular pressure , demonstrating the dynamic nature of actin within VSM and implying a shift in the F : G equilibrium in favor of F-actin .
	manualset3
229340	7	421424	7	NULL	NULL	0	NULL	VSM	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ) The cytosolic concentration of G-actin is significantly reduced by an elevation in intravascular pressure , demonstrating the dynamic nature of actin within VSM and implying a shift in the F : G equilibrium in favor of F-actin .
	manualset3
229341	8	421424	7	NULL	NULL	0	NULL	 shift 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ) The cytosolic concentration of G-actin is significantly reduced by an elevation in intravascular pressure , demonstrating the dynamic nature of actin within VSM and implying a shift in the F : G equilibrium in favor of F-actin .
	manualset3
229342	9	421424	7	NULL	NULL	0	NULL	F : G equilibrium	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ) The cytosolic concentration of G-actin is significantly reduced by an elevation in intravascular pressure , demonstrating the dynamic nature of actin within VSM and implying a shift in the F : G equilibrium in favor of F-actin .
	manualset3
229343	10	421424	7	NULL	NULL	0	NULL	 favor	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ) The cytosolic concentration of G-actin is significantly reduced by an elevation in intravascular pressure , demonstrating the dynamic nature of actin within VSM and implying a shift in the F : G equilibrium in favor of F-actin .
	manualset3
229344	11	421424	7	NULL	NULL	0	NULL	F-actin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	2 ) The cytosolic concentration of G-actin is significantly reduced by an elevation in intravascular pressure , demonstrating the dynamic nature of actin within VSM and implying a shift in the F : G equilibrium in favor of F-actin .
	manualset3
229345	1	421425	7	NULL	NULL	0	NULL	mixed infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In mixed infections with LDV-P and LDV-vx , LDV-C and LDV-v became rapidly lost even when present initially in large excess over the former .
	manualset3
229346	2	421425	7	NULL	NULL	0	NULL	LDV-P	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In mixed infections with LDV-P and LDV-vx , LDV-C and LDV-v became rapidly lost even when present initially in large excess over the former .
	manualset3
229347	3	421425	7	NULL	NULL	0	NULL	LDV-vx	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In mixed infections with LDV-P and LDV-vx , LDV-C and LDV-v became rapidly lost even when present initially in large excess over the former .
	manualset3
229348	4	421425	7	NULL	NULL	0	NULL	LDV-C	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In mixed infections with LDV-P and LDV-vx , LDV-C and LDV-v became rapidly lost even when present initially in large excess over the former .
	manualset3
229349	5	421425	7	NULL	NULL	0	NULL	LDV-v 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In mixed infections with LDV-P and LDV-vx , LDV-C and LDV-v became rapidly lost even when present initially in large excess over the former .
	manualset3
229350	6	421425	7	NULL	NULL	0	NULL	large excess 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In mixed infections with LDV-P and LDV-vx , LDV-C and LDV-v became rapidly lost even when present initially in large excess over the former .
	manualset3
229351	1	421426	7	NULL	NULL	0	NULL	flotillin-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we demonstrate that flotillin-1 , but not flotillin-2 , associates with lipid droplets upon oleic acid treatment and that this association is completely independent of caveolin .
	manualset3
229352	2	421426	7	NULL	NULL	0	NULL	flotillin-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we demonstrate that flotillin-1 , but not flotillin-2 , associates with lipid droplets upon oleic acid treatment and that this association is completely independent of caveolin .
	manualset3
229353	3	421426	7	NULL	NULL	0	NULL	lipid droplets	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we demonstrate that flotillin-1 , but not flotillin-2 , associates with lipid droplets upon oleic acid treatment and that this association is completely independent of caveolin .
	manualset3
229354	4	421426	7	NULL	NULL	0	NULL	 oleic acid treatment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we demonstrate that flotillin-1 , but not flotillin-2 , associates with lipid droplets upon oleic acid treatment and that this association is completely independent of caveolin .
	manualset3
229355	5	421426	7	NULL	NULL	NULL	NULL	 association	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Moreover , we demonstrate that flotillin-1 , but not flotillin-2 , associates with lipid droplets upon oleic acid treatment and that this association is completely independent of caveolin .
	manualset3
229356	6	421426	7	NULL	NULL	0	NULL	caveolin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , we demonstrate that flotillin-1 , but not flotillin-2 , associates with lipid droplets upon oleic acid treatment and that this association is completely independent of caveolin .
	manualset3
229357	1	421427	7	NULL	NULL	0	NULL	reference values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With optimized reference values , FQRSD , TQRSD and ISCSD contributed significantly to the identification of MVT patients and FQRSD to VF patients .
	manualset3
229358	2	421427	7	NULL	NULL	0	NULL	optimized reference values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With optimized reference values , FQRSD , TQRSD and ISCSD contributed significantly to the identification of MVT patients and FQRSD to VF patients .
	manualset3
229359	3	421427	7	NULL	NULL	0	NULL	FQRSD	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With optimized reference values , FQRSD , TQRSD and ISCSD contributed significantly to the identification of MVT patients and FQRSD to VF patients .
	manualset3
229360	4	421427	7	NULL	NULL	0	NULL	TQRSD	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With optimized reference values , FQRSD , TQRSD and ISCSD contributed significantly to the identification of MVT patients and FQRSD to VF patients .
	manualset3
229361	5	421427	7	NULL	NULL	0	NULL	ISCSD	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With optimized reference values , FQRSD , TQRSD and ISCSD contributed significantly to the identification of MVT patients and FQRSD to VF patients .
	manualset3
229362	6	421427	7	NULL	NULL	0	NULL	 identification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	With optimized reference values , FQRSD , TQRSD and ISCSD contributed significantly to the identification of MVT patients and FQRSD to VF patients .
	manualset3
229363	7	421427	7	NULL	NULL	0	NULL	MVT patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	With optimized reference values , FQRSD , TQRSD and ISCSD contributed significantly to the identification of MVT patients and FQRSD to VF patients .
	manualset3
229364	8	421427	7	NULL	NULL	0	NULL	FQRSD 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	With optimized reference values , FQRSD , TQRSD and ISCSD contributed significantly to the identification of MVT patients and FQRSD to VF patients .
	manualset3
229365	9	421427	7	NULL	NULL	0	NULL	VF patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	With optimized reference values , FQRSD , TQRSD and ISCSD contributed significantly to the identification of MVT patients and FQRSD to VF patients .
	manualset3
229366	1	421428	7	NULL	NULL	0	NULL	Insulin-like growth factors ( IGFs ) I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-like growth factors ( IGFs ) I and II are important regulators of cell proliferation and differentiation .
	manualset3
229367	2	421428	7	NULL	NULL	0	NULL	Insulin-like growth factors ( IGFs ) II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-like growth factors ( IGFs ) I and II are important regulators of cell proliferation and differentiation .
	manualset3
229368	3	421428	7	NULL	NULL	0	NULL	regulators	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-like growth factors ( IGFs ) I and II are important regulators of cell proliferation and differentiation .
	manualset3
229369	4	421428	7	NULL	NULL	0	NULL	cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-like growth factors ( IGFs ) I and II are important regulators of cell proliferation and differentiation .
	manualset3
229370	5	421428	7	NULL	NULL	0	NULL	differentiation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Insulin-like growth factors ( IGFs ) I and II are important regulators of cell proliferation and differentiation .
	manualset3
229371	1	421429	7	NULL	NULL	0	NULL	tetramer	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	For the tetramer of horseshoes ( 5 ) , quantum Monte Carlo calculations were used to fit the magnetic susceptibility behavior , giving two exchange interactions within the horseshoe ( -1.32 and -1.65 meV ) and a weak inter-horseshoe coupling of +0.12 meV .
	manualset3
229372	2	421429	7	NULL	NULL	0	NULL	horseshoes 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the tetramer of horseshoes ( 5 ) , quantum Monte Carlo calculations were used to fit the magnetic susceptibility behavior , giving two exchange interactions within the horseshoe ( -1.32 and -1.65 meV ) and a weak inter-horseshoe coupling of +0.12 meV .
	manualset3
229373	3	421429	7	NULL	NULL	0	NULL	quantum Monte Carlo calculations 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	For the tetramer of horseshoes ( 5 ) , quantum Monte Carlo calculations were used to fit the magnetic susceptibility behavior , giving two exchange interactions within the horseshoe ( -1.32 and -1.65 meV ) and a weak inter-horseshoe coupling of +0.12 meV .
	manualset3
229374	4	421429	7	NULL	NULL	0	NULL	magnetic susceptibility behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For the tetramer of horseshoes ( 5 ) , quantum Monte Carlo calculations were used to fit the magnetic susceptibility behavior , giving two exchange interactions within the horseshoe ( -1.32 and -1.65 meV ) and a weak inter-horseshoe coupling of +0.12 meV .
	manualset3
229375	5	421429	7	NULL	NULL	0	NULL	two exchange interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For the tetramer of horseshoes ( 5 ) , quantum Monte Carlo calculations were used to fit the magnetic susceptibility behavior , giving two exchange interactions within the horseshoe ( -1.32 and -1.65 meV ) and a weak inter-horseshoe coupling of +0.12 meV .
	manualset3
229376	6	421429	7	NULL	NULL	0	NULL	horseshoe 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the tetramer of horseshoes ( 5 ) , quantum Monte Carlo calculations were used to fit the magnetic susceptibility behavior , giving two exchange interactions within the horseshoe ( -1.32 and -1.65 meV ) and a weak inter-horseshoe coupling of +0.12 meV .
	manualset3
229377	7	421429	7	NULL	NULL	0	NULL	 -1.32 meV	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the tetramer of horseshoes ( 5 ) , quantum Monte Carlo calculations were used to fit the magnetic susceptibility behavior , giving two exchange interactions within the horseshoe ( -1.32 and -1.65 meV ) and a weak inter-horseshoe coupling of +0.12 meV .
	manualset3
229378	8	421429	7	NULL	NULL	0	NULL	 -1.65 meV	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the tetramer of horseshoes ( 5 ) , quantum Monte Carlo calculations were used to fit the magnetic susceptibility behavior , giving two exchange interactions within the horseshoe ( -1.32 and -1.65 meV ) and a weak inter-horseshoe coupling of +0.12 meV .
	manualset3
229379	9	421429	7	NULL	NULL	0	NULL	weak inter-horseshoe coupling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For the tetramer of horseshoes ( 5 ) , quantum Monte Carlo calculations were used to fit the magnetic susceptibility behavior , giving two exchange interactions within the horseshoe ( -1.32 and -1.65 meV ) and a weak inter-horseshoe coupling of +0.12 meV .
	manualset3
229380	10	421429	7	NULL	NULL	0	NULL	+0.12 meV	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the tetramer of horseshoes ( 5 ) , quantum Monte Carlo calculations were used to fit the magnetic susceptibility behavior , giving two exchange interactions within the horseshoe ( -1.32 and -1.65 meV ) and a weak inter-horseshoe coupling of +0.12 meV .
	manualset3
229381	1	421430	7	NULL	NULL	0	NULL	experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present experiments investigated the neurochemical bases of the rewarding properties of testosterone , focusing on the role of dopaminergic function in the acquisition of a testosterone conditioned place preference ( CPP ) .
	manualset3
229382	2	421430	7	NULL	NULL	0	NULL	neurochemical bases	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present experiments investigated the neurochemical bases of the rewarding properties of testosterone , focusing on the role of dopaminergic function in the acquisition of a testosterone conditioned place preference ( CPP ) .
	manualset3
229383	3	421430	7	NULL	NULL	0	NULL	rewarding properties	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present experiments investigated the neurochemical bases of the rewarding properties of testosterone , focusing on the role of dopaminergic function in the acquisition of a testosterone conditioned place preference ( CPP ) .
	manualset3
229384	4	421430	7	NULL	NULL	0	NULL	 role 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present experiments investigated the neurochemical bases of the rewarding properties of testosterone , focusing on the role of dopaminergic function in the acquisition of a testosterone conditioned place preference ( CPP ) .
	manualset3
229385	5	421430	7	NULL	NULL	0	NULL	dopaminergic function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present experiments investigated the neurochemical bases of the rewarding properties of testosterone , focusing on the role of dopaminergic function in the acquisition of a testosterone conditioned place preference ( CPP ) .
	manualset3
229386	6	421430	7	NULL	NULL	0	NULL	acquisition 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present experiments investigated the neurochemical bases of the rewarding properties of testosterone , focusing on the role of dopaminergic function in the acquisition of a testosterone conditioned place preference ( CPP ) .
	manualset3
229387	7	421430	7	NULL	NULL	0	NULL	testosterone 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present experiments investigated the neurochemical bases of the rewarding properties of testosterone , focusing on the role of dopaminergic function in the acquisition of a testosterone conditioned place preference ( CPP ) .
	manualset3
229388	8	421430	7	NULL	NULL	0	NULL	conditioned place preference ( CPP )	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present experiments investigated the neurochemical bases of the rewarding properties of testosterone , focusing on the role of dopaminergic function in the acquisition of a testosterone conditioned place preference ( CPP ) .
	manualset3
229389	9	421430	7	NULL	NULL	0	NULL	testosterone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The present experiments investigated the neurochemical bases of the rewarding properties of testosterone , focusing on the role of dopaminergic function in the acquisition of a testosterone conditioned place preference ( CPP ) .
	manualset3
229390	1	421431	7	NULL	NULL	0	NULL	acute dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An acute dose of gamma-hydroxybutyric acid alters gene expression in multiple mouse brain regions .
	manualset3
229391	2	421431	7	NULL	NULL	0	NULL	 gamma-hydroxybutyric acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An acute dose of gamma-hydroxybutyric acid alters gene expression in multiple mouse brain regions .
	manualset3
229392	3	421431	7	NULL	NULL	0	NULL	gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An acute dose of gamma-hydroxybutyric acid alters gene expression in multiple mouse brain regions .
	manualset3
229393	4	421431	7	NULL	NULL	0	NULL	multiple mouse brain regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An acute dose of gamma-hydroxybutyric acid alters gene expression in multiple mouse brain regions .
	manualset3
229394	1	421432	7	NULL	NULL	0	NULL	 lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histologically , the lesion showed proliferation of histiocytes in the fibroblastic background with formation of reactive germinal centers and many plasma cells .
	manualset3
229395	2	421432	7	NULL	NULL	0	NULL	proliferation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Histologically , the lesion showed proliferation of histiocytes in the fibroblastic background with formation of reactive germinal centers and many plasma cells .
	manualset3
229396	3	421432	7	NULL	NULL	0	NULL	histiocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Histologically , the lesion showed proliferation of histiocytes in the fibroblastic background with formation of reactive germinal centers and many plasma cells .
	manualset3
229397	4	421432	7	NULL	NULL	0	NULL	 fibroblastic background 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Histologically , the lesion showed proliferation of histiocytes in the fibroblastic background with formation of reactive germinal centers and many plasma cells .
	manualset3
229398	5	421432	7	NULL	NULL	NULL	NULL	formation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Histologically , the lesion showed proliferation of histiocytes in the fibroblastic background with formation of reactive germinal centers and many plasma cells .
	manualset3
229399	6	421432	7	NULL	NULL	0	NULL	 reactive germinal centers	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Histologically , the lesion showed proliferation of histiocytes in the fibroblastic background with formation of reactive germinal centers and many plasma cells .
	manualset3
229400	7	421432	7	NULL	NULL	0	NULL	 plasma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Histologically , the lesion showed proliferation of histiocytes in the fibroblastic background with formation of reactive germinal centers and many plasma cells .
	manualset3
229401	1	421433	7	NULL	NULL	0	NULL	Na + ingress	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Resulting Na + ingress may cause sustained partial depolarization , cytoplasmic alkalinization , and initiation of cell cycling .
	manualset3
229402	2	421433	7	NULL	NULL	0	NULL	sustained partial depolarization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Resulting Na + ingress may cause sustained partial depolarization , cytoplasmic alkalinization , and initiation of cell cycling .
	manualset3
229403	3	421433	7	NULL	NULL	0	NULL	cytoplasmic alkalinization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Resulting Na + ingress may cause sustained partial depolarization , cytoplasmic alkalinization , and initiation of cell cycling .
	manualset3
229404	4	421433	7	NULL	NULL	0	NULL	initiation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Resulting Na + ingress may cause sustained partial depolarization , cytoplasmic alkalinization , and initiation of cell cycling .
	manualset3
229405	5	421433	7	NULL	NULL	0	NULL	cell cycling	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Resulting Na + ingress may cause sustained partial depolarization , cytoplasmic alkalinization , and initiation of cell cycling .
	manualset3
229406	1	421434	7	NULL	NULL	0	NULL	conclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the expression of ERBB2 in prostate cancer is relatively low , and is not altered during disease progression .
	manualset3
229407	2	421434	7	NULL	NULL	0	NULL	 expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the expression of ERBB2 in prostate cancer is relatively low , and is not altered during disease progression .
	manualset3
229408	3	421434	7	NULL	NULL	0	NULL	ERBB2	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the expression of ERBB2 in prostate cancer is relatively low , and is not altered during disease progression .
	manualset3
229409	4	421434	7	NULL	NULL	0	NULL	prostate cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the expression of ERBB2 in prostate cancer is relatively low , and is not altered during disease progression .
	manualset3
229410	5	421434	7	NULL	NULL	0	NULL	disease progression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the expression of ERBB2 in prostate cancer is relatively low , and is not altered during disease progression .
	manualset3
229517	1	421435	7	NULL	NULL	0	NULL	 effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effect of laser radiation on the teeth and soft tissues of the oral cavity ) .
	manualset3
229518	2	421435	7	NULL	NULL	0	NULL	 laser radiation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effect of laser radiation on the teeth and soft tissues of the oral cavity ) .
	manualset3
229519	3	421435	7	NULL	NULL	0	NULL	teeth	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effect of laser radiation on the teeth and soft tissues of the oral cavity ) .
	manualset3
229520	4	421435	7	NULL	NULL	0	NULL	 soft tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effect of laser radiation on the teeth and soft tissues of the oral cavity ) .
	manualset3
229521	5	421435	7	NULL	NULL	0	NULL	oral cavity	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effect of laser radiation on the teeth and soft tissues of the oral cavity ) .
	manualset3
229522	1	421436	7	NULL	NULL	0	NULL	Sleep disruption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep disruption was reflected in reduced time spent asleep , and in changed REM latency , which increased in the phase advance direction but decreased in the phase delay direction .
	manualset3
229523	2	421436	7	NULL	NULL	0	NULL	reduced time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep disruption was reflected in reduced time spent asleep , and in changed REM latency , which increased in the phase advance direction but decreased in the phase delay direction .
	manualset3
229524	3	421436	7	NULL	NULL	0	NULL	asleep	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep disruption was reflected in reduced time spent asleep , and in changed REM latency , which increased in the phase advance direction but decreased in the phase delay direction .
	manualset3
229525	4	421436	7	NULL	NULL	0	NULL	changed REM latency	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep disruption was reflected in reduced time spent asleep , and in changed REM latency , which increased in the phase advance direction but decreased in the phase delay direction .
	manualset3
229526	5	421436	7	NULL	NULL	0	NULL	phase advance direction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep disruption was reflected in reduced time spent asleep , and in changed REM latency , which increased in the phase advance direction but decreased in the phase delay direction .
	manualset3
229527	6	421436	7	NULL	NULL	0	NULL	phase delay direction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep disruption was reflected in reduced time spent asleep , and in changed REM latency , which increased in the phase advance direction but decreased in the phase delay direction .
	manualset3
229528	1	421437	7	NULL	NULL	0	NULL	magnitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably , the magnitude of the precue activity varied across the four blocks of the one-direction-rewarded ( 1DR ) condition , depending on which direction was rewarded .
	manualset3
229529	2	421437	7	NULL	NULL	0	NULL	precue activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably , the magnitude of the precue activity varied across the four blocks of the one-direction-rewarded ( 1DR ) condition , depending on which direction was rewarded .
	manualset3
229530	3	421437	7	NULL	NULL	0	NULL	 four blocks	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably , the magnitude of the precue activity varied across the four blocks of the one-direction-rewarded ( 1DR ) condition , depending on which direction was rewarded .
	manualset3
229531	4	421437	7	NULL	NULL	0	NULL	one-direction-rewarded ( 1DR ) condition 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably , the magnitude of the precue activity varied across the four blocks of the one-direction-rewarded ( 1DR ) condition , depending on which direction was rewarded .
	manualset3
229532	5	421437	7	NULL	NULL	0	NULL	direction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Remarkably , the magnitude of the precue activity varied across the four blocks of the one-direction-rewarded ( 1DR ) condition , depending on which direction was rewarded .
	manualset3
229533	1	421438	7	NULL	NULL	0	NULL	Aldosterone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Aldosterone produced a small compensation while corticosterone produced a compensation similar to that seen in sham-operated animals .
	manualset3
229534	2	421438	7	NULL	NULL	0	NULL	small compensation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Aldosterone produced a small compensation while corticosterone produced a compensation similar to that seen in sham-operated animals .
	manualset3
229535	3	421438	7	NULL	NULL	0	NULL	corticosterone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Aldosterone produced a small compensation while corticosterone produced a compensation similar to that seen in sham-operated animals .
	manualset3
229536	4	421438	7	NULL	NULL	0	NULL	compensation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Aldosterone produced a small compensation while corticosterone produced a compensation similar to that seen in sham-operated animals .
	manualset3
229537	5	421438	7	NULL	NULL	0	NULL	sham-operated animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Aldosterone produced a small compensation while corticosterone produced a compensation similar to that seen in sham-operated animals .
	manualset3
229538	1	421439	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , activation of ERKs , members of the mitogen-activated protein kinase family , by isoproterenol was examined in a human salivary gland cell line ( HSY ) .
	manualset3
229539	2	421439	7	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , activation of ERKs , members of the mitogen-activated protein kinase family , by isoproterenol was examined in a human salivary gland cell line ( HSY ) .
	manualset3
229540	3	421439	7	NULL	NULL	0	NULL	ERKs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , activation of ERKs , members of the mitogen-activated protein kinase family , by isoproterenol was examined in a human salivary gland cell line ( HSY ) .
	manualset3
229541	4	421439	7	NULL	NULL	0	NULL	members	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , activation of ERKs , members of the mitogen-activated protein kinase family , by isoproterenol was examined in a human salivary gland cell line ( HSY ) .
	manualset3
229542	5	421439	7	NULL	NULL	0	NULL	mitogen-activated protein kinase family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , activation of ERKs , members of the mitogen-activated protein kinase family , by isoproterenol was examined in a human salivary gland cell line ( HSY ) .
	manualset3
229543	6	421439	7	NULL	NULL	0	NULL	 isoproterenol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , activation of ERKs , members of the mitogen-activated protein kinase family , by isoproterenol was examined in a human salivary gland cell line ( HSY ) .
	manualset3
229544	7	421439	7	NULL	NULL	0	NULL	human salivary gland cell line ( HSY ) 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , activation of ERKs , members of the mitogen-activated protein kinase family , by isoproterenol was examined in a human salivary gland cell line ( HSY ) .
	manualset3
229545	1	421440	7	NULL	NULL	0	NULL	Evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluation of the cellular contents of the injection site is a much better indicator of the immunomodulatory effects of lutein than measurements of the amount of swelling .
	manualset3
229546	2	421440	7	NULL	NULL	0	NULL	cellular contents 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluation of the cellular contents of the injection site is a much better indicator of the immunomodulatory effects of lutein than measurements of the amount of swelling .
	manualset3
229547	3	421440	7	NULL	NULL	0	NULL	injection site	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluation of the cellular contents of the injection site is a much better indicator of the immunomodulatory effects of lutein than measurements of the amount of swelling .
	manualset3
229548	4	421440	7	NULL	NULL	0	NULL	indicator 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluation of the cellular contents of the injection site is a much better indicator of the immunomodulatory effects of lutein than measurements of the amount of swelling .
	manualset3
229549	5	421440	7	NULL	NULL	0	NULL	immunomodulatory effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluation of the cellular contents of the injection site is a much better indicator of the immunomodulatory effects of lutein than measurements of the amount of swelling .
	manualset3
229550	6	421440	7	NULL	NULL	0	NULL	lutein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluation of the cellular contents of the injection site is a much better indicator of the immunomodulatory effects of lutein than measurements of the amount of swelling .
	manualset3
229551	7	421440	7	NULL	NULL	NULL	NULL	measurements	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Evaluation of the cellular contents of the injection site is a much better indicator of the immunomodulatory effects of lutein than measurements of the amount of swelling .
	manualset3
229552	8	421440	7	NULL	NULL	0	NULL	amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluation of the cellular contents of the injection site is a much better indicator of the immunomodulatory effects of lutein than measurements of the amount of swelling .
	manualset3
229553	9	421440	7	NULL	NULL	0	NULL	swelling	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Evaluation of the cellular contents of the injection site is a much better indicator of the immunomodulatory effects of lutein than measurements of the amount of swelling .
	manualset3
229554	1	421441	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with lesions above the 5th vertebra , not only the voluntary movements of the elbow are restricted , but also the overall number of preserved movements available for control purposes decreases .
	manualset3
229555	2	421441	7	NULL	NULL	0	NULL	lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with lesions above the 5th vertebra , not only the voluntary movements of the elbow are restricted , but also the overall number of preserved movements available for control purposes decreases .
	manualset3
229556	3	421441	7	NULL	NULL	0	NULL	5th vertebra	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with lesions above the 5th vertebra , not only the voluntary movements of the elbow are restricted , but also the overall number of preserved movements available for control purposes decreases .
	manualset3
229557	4	421441	7	NULL	NULL	0	NULL	voluntary movements	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with lesions above the 5th vertebra , not only the voluntary movements of the elbow are restricted , but also the overall number of preserved movements available for control purposes decreases .
	manualset3
229558	5	421441	7	NULL	NULL	0	NULL	 elbow	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with lesions above the 5th vertebra , not only the voluntary movements of the elbow are restricted , but also the overall number of preserved movements available for control purposes decreases .
	manualset3
229559	6	421441	7	NULL	NULL	0	NULL	overall number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with lesions above the 5th vertebra , not only the voluntary movements of the elbow are restricted , but also the overall number of preserved movements available for control purposes decreases .
	manualset3
229560	7	421441	7	NULL	NULL	0	NULL	preserved movements	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with lesions above the 5th vertebra , not only the voluntary movements of the elbow are restricted , but also the overall number of preserved movements available for control purposes decreases .
	manualset3
229561	8	421441	7	NULL	NULL	0	NULL	control purposes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In patients with lesions above the 5th vertebra , not only the voluntary movements of the elbow are restricted , but also the overall number of preserved movements available for control purposes decreases .
	manualset3
229562	1	421442	7	NULL	NULL	0	NULL	adrenoceptor-antagonist	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An adrenoceptor-antagonist , such as yohimbine , phentolamine , prazosin or corynanthine was injected into the NTS of other anesthetized rabbits .
	manualset3
229563	2	421442	7	NULL	NULL	0	NULL	yohimbine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An adrenoceptor-antagonist , such as yohimbine , phentolamine , prazosin or corynanthine was injected into the NTS of other anesthetized rabbits .
	manualset3
229564	3	421442	7	NULL	NULL	0	NULL	phentolamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An adrenoceptor-antagonist , such as yohimbine , phentolamine , prazosin or corynanthine was injected into the NTS of other anesthetized rabbits .
	manualset3
229565	4	421442	7	NULL	NULL	0	NULL	 prazosin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An adrenoceptor-antagonist , such as yohimbine , phentolamine , prazosin or corynanthine was injected into the NTS of other anesthetized rabbits .
	manualset3
229566	5	421442	7	NULL	NULL	0	NULL	corynanthine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An adrenoceptor-antagonist , such as yohimbine , phentolamine , prazosin or corynanthine was injected into the NTS of other anesthetized rabbits .
	manualset3
229567	6	421442	7	NULL	NULL	0	NULL	NTS	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	An adrenoceptor-antagonist , such as yohimbine , phentolamine , prazosin or corynanthine was injected into the NTS of other anesthetized rabbits .
	manualset3
229568	7	421442	7	NULL	NULL	0	NULL	anesthetized rabbits	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	An adrenoceptor-antagonist , such as yohimbine , phentolamine , prazosin or corynanthine was injected into the NTS of other anesthetized rabbits .
	manualset3
229569	1	421443	7	NULL	NULL	0	NULL	Biological expediency 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Biological expediency of discrimination between potassium and sodium by cells ) .
	manualset3
229570	2	421443	7	NULL	NULL	0	NULL	discrimination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Biological expediency of discrimination between potassium and sodium by cells ) .
	manualset3
229571	3	421443	7	NULL	NULL	0	NULL	potassium 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Biological expediency of discrimination between potassium and sodium by cells ) .
	manualset3
229572	4	421443	7	NULL	NULL	0	NULL	 sodium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Biological expediency of discrimination between potassium and sodium by cells ) .
	manualset3
229573	5	421443	7	NULL	NULL	0	NULL	cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	( Biological expediency of discrimination between potassium and sodium by cells ) .
	manualset3
229574	1	421444	7	NULL	NULL	0	NULL	thermophilic , sulfate-reducing bacterium	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A thermophilic , sulfate-reducing bacterium , strain MT-96T , was isolated from an active , marine , shallow-water hydrothermal vent system .
	manualset3
229575	2	421444	7	NULL	NULL	0	NULL	strain MT-96T	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A thermophilic , sulfate-reducing bacterium , strain MT-96T , was isolated from an active , marine , shallow-water hydrothermal vent system .
	manualset3
229576	3	421444	7	NULL	NULL	0	NULL	active , marine , shallow-water hydrothermal vent system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	A thermophilic , sulfate-reducing bacterium , strain MT-96T , was isolated from an active , marine , shallow-water hydrothermal vent system .
	manualset3
229577	1	421445	7	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effect of storage conditions and containers on the biochemical content of Fructus anis ) .
	manualset3
229578	2	421445	7	NULL	NULL	0	NULL	storage conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effect of storage conditions and containers on the biochemical content of Fructus anis ) .
	manualset3
229579	3	421445	7	NULL	NULL	0	NULL	containers	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effect of storage conditions and containers on the biochemical content of Fructus anis ) .
	manualset3
229580	4	421445	7	NULL	NULL	0	NULL	biochemical content 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effect of storage conditions and containers on the biochemical content of Fructus anis ) .
	manualset3
229581	5	421445	7	NULL	NULL	0	NULL	Fructus anis 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( The effect of storage conditions and containers on the biochemical content of Fructus anis ) .
	manualset3
229582	1	421446	7	NULL	NULL	0	NULL	Genetic analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic analysis revealed that full expression of the hypermuscular phenotype requires the action of modifier loci in addition to Mstn ( Cmpt-dl1Abc ) .
	manualset3
229583	2	421446	7	NULL	NULL	0	NULL	full expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic analysis revealed that full expression of the hypermuscular phenotype requires the action of modifier loci in addition to Mstn ( Cmpt-dl1Abc ) .
	manualset3
229584	3	421446	7	NULL	NULL	0	NULL	hypermuscular phenotype 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic analysis revealed that full expression of the hypermuscular phenotype requires the action of modifier loci in addition to Mstn ( Cmpt-dl1Abc ) .
	manualset3
229585	4	421446	7	NULL	NULL	0	NULL	 action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic analysis revealed that full expression of the hypermuscular phenotype requires the action of modifier loci in addition to Mstn ( Cmpt-dl1Abc ) .
	manualset3
229586	5	421446	7	NULL	NULL	0	NULL	modifier loci 	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic analysis revealed that full expression of the hypermuscular phenotype requires the action of modifier loci in addition to Mstn ( Cmpt-dl1Abc ) .
	manualset3
229587	6	421446	7	NULL	NULL	0	NULL	Mstn ( Cmpt-dl1Abc )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Genetic analysis revealed that full expression of the hypermuscular phenotype requires the action of modifier loci in addition to Mstn ( Cmpt-dl1Abc ) .
	manualset3
229588	1	421447	7	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study semiquantitative reverse transcriptase polymerase chain reaction ( PCR ) is compared with a new branched DNA signal amplification methodology .
	manualset3
229589	2	421447	7	NULL	NULL	0	NULL	semiquantitative reverse transcriptase polymerase chain reaction ( PCR )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study semiquantitative reverse transcriptase polymerase chain reaction ( PCR ) is compared with a new branched DNA signal amplification methodology .
	manualset3
229590	3	421447	7	NULL	NULL	0	NULL	new branched DNA signal amplification methodology 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study semiquantitative reverse transcriptase polymerase chain reaction ( PCR ) is compared with a new branched DNA signal amplification methodology .
	manualset3
229591	1	421448	7	NULL	NULL	NULL	NULL	adaption	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An adaption of the selection or the time of administration of antihypertensive drugs with respect to the circadian rhythm is beneficial to control blood pressure and reduce cardiovascular morbidity .
	manualset3
229592	2	421448	7	NULL	NULL	0	NULL	 selection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An adaption of the selection or the time of administration of antihypertensive drugs with respect to the circadian rhythm is beneficial to control blood pressure and reduce cardiovascular morbidity .
	manualset3
229593	3	421448	7	NULL	NULL	0	NULL	administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An adaption of the selection or the time of administration of antihypertensive drugs with respect to the circadian rhythm is beneficial to control blood pressure and reduce cardiovascular morbidity .
	manualset3
229594	4	421448	7	NULL	NULL	0	NULL	antihypertensive drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	An adaption of the selection or the time of administration of antihypertensive drugs with respect to the circadian rhythm is beneficial to control blood pressure and reduce cardiovascular morbidity .
	manualset3
229595	5	421448	7	NULL	NULL	0	NULL	circadian rhythm	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An adaption of the selection or the time of administration of antihypertensive drugs with respect to the circadian rhythm is beneficial to control blood pressure and reduce cardiovascular morbidity .
	manualset3
229596	6	421448	7	NULL	NULL	0	NULL	blood pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An adaption of the selection or the time of administration of antihypertensive drugs with respect to the circadian rhythm is beneficial to control blood pressure and reduce cardiovascular morbidity .
	manualset3
229597	7	421448	7	NULL	NULL	0	NULL	cardiovascular morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An adaption of the selection or the time of administration of antihypertensive drugs with respect to the circadian rhythm is beneficial to control blood pressure and reduce cardiovascular morbidity .
	manualset3
229598	8	421448	7	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	An adaption of the selection or the time of administration of antihypertensive drugs with respect to the circadian rhythm is beneficial to control blood pressure and reduce cardiovascular morbidity .
	manualset3
229599	1	421449	7	NULL	NULL	0	NULL	Bromodeoxyuridine ( BUdR )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Bromodeoxyuridine ( BUdR ) is a non-radioactive thymidine analog which is incorporated into DNA during the S-phase of cycling cells .
	manualset3
229600	2	421449	7	NULL	NULL	0	NULL	non-radioactive thymidine analog	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Bromodeoxyuridine ( BUdR ) is a non-radioactive thymidine analog which is incorporated into DNA during the S-phase of cycling cells .
	manualset3
229601	3	421449	7	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Bromodeoxyuridine ( BUdR ) is a non-radioactive thymidine analog which is incorporated into DNA during the S-phase of cycling cells .
	manualset3
229602	4	421449	7	NULL	NULL	0	NULL	S-phase	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Bromodeoxyuridine ( BUdR ) is a non-radioactive thymidine analog which is incorporated into DNA during the S-phase of cycling cells .
	manualset3
229603	5	421449	7	NULL	NULL	0	NULL	cycling cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Bromodeoxyuridine ( BUdR ) is a non-radioactive thymidine analog which is incorporated into DNA during the S-phase of cycling cells .
	manualset3
229604	1	421450	7	NULL	NULL	0	NULL	immunochemistry	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunochemistry of toxins and toxoids ; the solubility of staphylococcal toxin in methanol-water mixtures under controlled conditions of pH , ionic strength , and temperature .
	manualset3
229605	2	421450	7	NULL	NULL	0	NULL	toxins	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunochemistry of toxins and toxoids ; the solubility of staphylococcal toxin in methanol-water mixtures under controlled conditions of pH , ionic strength , and temperature .
	manualset3
229606	3	421450	7	NULL	NULL	0	NULL	toxoids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunochemistry of toxins and toxoids ; the solubility of staphylococcal toxin in methanol-water mixtures under controlled conditions of pH , ionic strength , and temperature .
	manualset3
229607	4	421450	7	NULL	NULL	0	NULL	solubility	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunochemistry of toxins and toxoids ; the solubility of staphylococcal toxin in methanol-water mixtures under controlled conditions of pH , ionic strength , and temperature .
	manualset3
229608	5	421450	7	NULL	NULL	0	NULL	staphylococcal toxin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunochemistry of toxins and toxoids ; the solubility of staphylococcal toxin in methanol-water mixtures under controlled conditions of pH , ionic strength , and temperature .
	manualset3
229609	6	421450	7	NULL	NULL	0	NULL	methanol-water mixtures	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunochemistry of toxins and toxoids ; the solubility of staphylococcal toxin in methanol-water mixtures under controlled conditions of pH , ionic strength , and temperature .
	manualset3
229610	7	421450	7	NULL	NULL	0	NULL	controlled conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunochemistry of toxins and toxoids ; the solubility of staphylococcal toxin in methanol-water mixtures under controlled conditions of pH , ionic strength , and temperature .
	manualset3
229611	8	421450	7	NULL	NULL	0	NULL	 pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunochemistry of toxins and toxoids ; the solubility of staphylococcal toxin in methanol-water mixtures under controlled conditions of pH , ionic strength , and temperature .
	manualset3
229612	9	421450	7	NULL	NULL	0	NULL	 ionic strength 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunochemistry of toxins and toxoids ; the solubility of staphylococcal toxin in methanol-water mixtures under controlled conditions of pH , ionic strength , and temperature .
	manualset3
229613	10	421450	7	NULL	NULL	0	NULL	temperature	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunochemistry of toxins and toxoids ; the solubility of staphylococcal toxin in methanol-water mixtures under controlled conditions of pH , ionic strength , and temperature .
	manualset3
229614	1	421451	7	NULL	NULL	0	NULL	optical density	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The optical density of human rhodopsin in vivo is about 0.35 ( common logarithmic units ) at its gamma ( max . )
	manualset3
229615	2	421451	7	NULL	NULL	0	NULL	human rhodopsin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The optical density of human rhodopsin in vivo is about 0.35 ( common logarithmic units ) at its gamma ( max . )
	manualset3
229616	3	421451	7	NULL	NULL	0	NULL	0.35	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The optical density of human rhodopsin in vivo is about 0.35 ( common logarithmic units ) at its gamma ( max . )
	manualset3
229617	4	421451	7	NULL	NULL	0	NULL	common logarithmic units 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The optical density of human rhodopsin in vivo is about 0.35 ( common logarithmic units ) at its gamma ( max . )
	manualset3
229618	5	421451	7	NULL	NULL	0	NULL	gamma ( max  )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The optical density of human rhodopsin in vivo is about 0.35 ( common logarithmic units ) at its gamma ( max . )
	manualset3
229619	1	421452	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of an agonistic anti-Fas antibody ( Ab ) ( CH-11 ) to hematopoietic stem cell culture of BM cells more strongly suppressed colony formation from granulocyte-macrophage colony-forming units ( GM-CFU ) and erythroid burst-forming units ( BFU-E ) after BMT .
	manualset3
229620	2	421452	7	NULL	NULL	0	NULL	agonistic anti-Fas antibody ( Ab ) ( CH-11 )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of an agonistic anti-Fas antibody ( Ab ) ( CH-11 ) to hematopoietic stem cell culture of BM cells more strongly suppressed colony formation from granulocyte-macrophage colony-forming units ( GM-CFU ) and erythroid burst-forming units ( BFU-E ) after BMT .
	manualset3
229621	3	421452	7	NULL	NULL	0	NULL	hematopoietic stem cell culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of an agonistic anti-Fas antibody ( Ab ) ( CH-11 ) to hematopoietic stem cell culture of BM cells more strongly suppressed colony formation from granulocyte-macrophage colony-forming units ( GM-CFU ) and erythroid burst-forming units ( BFU-E ) after BMT .
	manualset3
229622	4	421452	7	NULL	NULL	0	NULL	BM cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of an agonistic anti-Fas antibody ( Ab ) ( CH-11 ) to hematopoietic stem cell culture of BM cells more strongly suppressed colony formation from granulocyte-macrophage colony-forming units ( GM-CFU ) and erythroid burst-forming units ( BFU-E ) after BMT .
	manualset3
229623	5	421452	7	NULL	NULL	0	NULL	colony formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of an agonistic anti-Fas antibody ( Ab ) ( CH-11 ) to hematopoietic stem cell culture of BM cells more strongly suppressed colony formation from granulocyte-macrophage colony-forming units ( GM-CFU ) and erythroid burst-forming units ( BFU-E ) after BMT .
	manualset3
229624	6	421452	7	NULL	NULL	0	NULL	granulocyte-macrophage colony-forming units ( GM-CFU ) 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of an agonistic anti-Fas antibody ( Ab ) ( CH-11 ) to hematopoietic stem cell culture of BM cells more strongly suppressed colony formation from granulocyte-macrophage colony-forming units ( GM-CFU ) and erythroid burst-forming units ( BFU-E ) after BMT .
	manualset3
229625	7	421452	7	NULL	NULL	0	NULL	erythroid burst-forming units ( BFU-E ) 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of an agonistic anti-Fas antibody ( Ab ) ( CH-11 ) to hematopoietic stem cell culture of BM cells more strongly suppressed colony formation from granulocyte-macrophage colony-forming units ( GM-CFU ) and erythroid burst-forming units ( BFU-E ) after BMT .
	manualset3
229626	8	421452	7	NULL	NULL	0	NULL	BMT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The addition of an agonistic anti-Fas antibody ( Ab ) ( CH-11 ) to hematopoietic stem cell culture of BM cells more strongly suppressed colony formation from granulocyte-macrophage colony-forming units ( GM-CFU ) and erythroid burst-forming units ( BFU-E ) after BMT .
	manualset3
229627	1	421453	7	NULL	NULL	0	NULL	adaptive implementation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An adaptive implementation of the spatial matched filter and its application to the reconstruction of phased array MR imagery is described .
	manualset3
229628	2	421453	7	NULL	NULL	0	NULL	spatial matched filter	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	An adaptive implementation of the spatial matched filter and its application to the reconstruction of phased array MR imagery is described .
	manualset3
229629	3	421453	7	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An adaptive implementation of the spatial matched filter and its application to the reconstruction of phased array MR imagery is described .
	manualset3
229630	4	421453	7	NULL	NULL	0	NULL	reconstruction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An adaptive implementation of the spatial matched filter and its application to the reconstruction of phased array MR imagery is described .
	manualset3
229631	5	421453	7	NULL	NULL	0	NULL	phased array MR imagery 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An adaptive implementation of the spatial matched filter and its application to the reconstruction of phased array MR imagery is described .
	manualset3
229632	1	421454	7	NULL	NULL	0	NULL	MD simulations	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	MD simulations show that the Thr729Lys mutation provokes a structural perturbation of the CPT-binding pocket .
	manualset3
229633	2	421454	7	NULL	NULL	0	NULL	Thr729Lys mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MD simulations show that the Thr729Lys mutation provokes a structural perturbation of the CPT-binding pocket .
	manualset3
229634	3	421454	7	NULL	NULL	0	NULL	structural perturbation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	MD simulations show that the Thr729Lys mutation provokes a structural perturbation of the CPT-binding pocket .
	manualset3
229635	4	421454	7	NULL	NULL	0	NULL	CPT-binding pocket	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	MD simulations show that the Thr729Lys mutation provokes a structural perturbation of the CPT-binding pocket .
	manualset3
229636	1	421455	7	NULL	NULL	0	NULL	Myometrium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Myometrium , endometrium , and placenta from Day 75 and Day 105 pregnant gilts were also evaluated for ALP and UF mRNA expression to determine regional expression of these steroid-regulated genes .
	manualset3
229637	2	421455	7	NULL	NULL	0	NULL	endometrium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Myometrium , endometrium , and placenta from Day 75 and Day 105 pregnant gilts were also evaluated for ALP and UF mRNA expression to determine regional expression of these steroid-regulated genes .
	manualset3
229638	3	421455	7	NULL	NULL	0	NULL	placenta	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Myometrium , endometrium , and placenta from Day 75 and Day 105 pregnant gilts were also evaluated for ALP and UF mRNA expression to determine regional expression of these steroid-regulated genes .
	manualset3
229639	4	421455	7	NULL	NULL	0	NULL	 Day 75 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Myometrium , endometrium , and placenta from Day 75 and Day 105 pregnant gilts were also evaluated for ALP and UF mRNA expression to determine regional expression of these steroid-regulated genes .
	manualset3
229640	5	421455	7	NULL	NULL	0	NULL	Day 105	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Myometrium , endometrium , and placenta from Day 75 and Day 105 pregnant gilts were also evaluated for ALP and UF mRNA expression to determine regional expression of these steroid-regulated genes .
	manualset3
229641	6	421455	7	NULL	NULL	0	NULL	pregnant gilts	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Myometrium , endometrium , and placenta from Day 75 and Day 105 pregnant gilts were also evaluated for ALP and UF mRNA expression to determine regional expression of these steroid-regulated genes .
	manualset3
229642	7	421455	7	NULL	NULL	0	NULL	ALP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Myometrium , endometrium , and placenta from Day 75 and Day 105 pregnant gilts were also evaluated for ALP and UF mRNA expression to determine regional expression of these steroid-regulated genes .
	manualset3
229643	8	421455	7	NULL	NULL	0	NULL	UF mRNA expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Myometrium , endometrium , and placenta from Day 75 and Day 105 pregnant gilts were also evaluated for ALP and UF mRNA expression to determine regional expression of these steroid-regulated genes .
	manualset3
229644	9	421455	7	NULL	NULL	0	NULL	 regional expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Myometrium , endometrium , and placenta from Day 75 and Day 105 pregnant gilts were also evaluated for ALP and UF mRNA expression to determine regional expression of these steroid-regulated genes .
	manualset3
229645	10	421455	7	NULL	NULL	0	NULL	steroid-regulated genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Myometrium , endometrium , and placenta from Day 75 and Day 105 pregnant gilts were also evaluated for ALP and UF mRNA expression to determine regional expression of these steroid-regulated genes .
	manualset3
229646	1	421456	7	NULL	NULL	0	NULL	HLA-restriction analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	HLA-restriction analysis showed that in addition to HLA-DRB1 products ( serologically defined HLA-DR1 to HLA-DR10 ) , the HLA molecules encoded by HLA-DRB3 ( HLA-DR52 ) and HLA-DRB4 ( HLA-DR53 ) are important in presentation of mycobacterial antigens and epitopes to T cells .
	manualset3
229647	2	421456	7	NULL	NULL	0	NULL	HLA-DRB1 products	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	HLA-restriction analysis showed that in addition to HLA-DRB1 products ( serologically defined HLA-DR1 to HLA-DR10 ) , the HLA molecules encoded by HLA-DRB3 ( HLA-DR52 ) and HLA-DRB4 ( HLA-DR53 ) are important in presentation of mycobacterial antigens and epitopes to T cells .
	manualset3
229648	3	421456	7	NULL	NULL	NULL	NULL	HLA-DR1 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	HLA-restriction analysis showed that in addition to HLA-DRB1 products ( serologically defined HLA-DR1 to HLA-DR10 ) , the HLA molecules encoded by HLA-DRB3 ( HLA-DR52 ) and HLA-DRB4 ( HLA-DR53 ) are important in presentation of mycobacterial antigens and epitopes to T cells .
	manualset3
229649	4	421456	7	NULL	NULL	NULL	NULL	HLA-DR10 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	HLA-restriction analysis showed that in addition to HLA-DRB1 products ( serologically defined HLA-DR1 to HLA-DR10 ) , the HLA molecules encoded by HLA-DRB3 ( HLA-DR52 ) and HLA-DRB4 ( HLA-DR53 ) are important in presentation of mycobacterial antigens and epitopes to T cells .
	manualset3
229650	5	421456	7	NULL	NULL	0	NULL	HLA molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	HLA-restriction analysis showed that in addition to HLA-DRB1 products ( serologically defined HLA-DR1 to HLA-DR10 ) , the HLA molecules encoded by HLA-DRB3 ( HLA-DR52 ) and HLA-DRB4 ( HLA-DR53 ) are important in presentation of mycobacterial antigens and epitopes to T cells .
	manualset3
229651	6	421456	7	NULL	NULL	NULL	NULL	HLA-DRB3 ( HLA-DR52 )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	HLA-restriction analysis showed that in addition to HLA-DRB1 products ( serologically defined HLA-DR1 to HLA-DR10 ) , the HLA molecules encoded by HLA-DRB3 ( HLA-DR52 ) and HLA-DRB4 ( HLA-DR53 ) are important in presentation of mycobacterial antigens and epitopes to T cells .
	manualset3
229652	7	421456	7	NULL	NULL	NULL	NULL	HLA-DRB4 ( HLA-DR53 )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	HLA-restriction analysis showed that in addition to HLA-DRB1 products ( serologically defined HLA-DR1 to HLA-DR10 ) , the HLA molecules encoded by HLA-DRB3 ( HLA-DR52 ) and HLA-DRB4 ( HLA-DR53 ) are important in presentation of mycobacterial antigens and epitopes to T cells .
	manualset3
229653	8	421456	7	NULL	NULL	0	NULL	presentation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HLA-restriction analysis showed that in addition to HLA-DRB1 products ( serologically defined HLA-DR1 to HLA-DR10 ) , the HLA molecules encoded by HLA-DRB3 ( HLA-DR52 ) and HLA-DRB4 ( HLA-DR53 ) are important in presentation of mycobacterial antigens and epitopes to T cells .
	manualset3
229654	9	421456	7	NULL	NULL	0	NULL	mycobacterial antigens	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	HLA-restriction analysis showed that in addition to HLA-DRB1 products ( serologically defined HLA-DR1 to HLA-DR10 ) , the HLA molecules encoded by HLA-DRB3 ( HLA-DR52 ) and HLA-DRB4 ( HLA-DR53 ) are important in presentation of mycobacterial antigens and epitopes to T cells .
	manualset3
229655	10	421456	7	NULL	NULL	0	NULL	epitopes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	HLA-restriction analysis showed that in addition to HLA-DRB1 products ( serologically defined HLA-DR1 to HLA-DR10 ) , the HLA molecules encoded by HLA-DRB3 ( HLA-DR52 ) and HLA-DRB4 ( HLA-DR53 ) are important in presentation of mycobacterial antigens and epitopes to T cells .
	manualset3
229656	11	421456	7	NULL	NULL	0	NULL	 T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	HLA-restriction analysis showed that in addition to HLA-DRB1 products ( serologically defined HLA-DR1 to HLA-DR10 ) , the HLA molecules encoded by HLA-DRB3 ( HLA-DR52 ) and HLA-DRB4 ( HLA-DR53 ) are important in presentation of mycobacterial antigens and epitopes to T cells .
	manualset3
229657	1	421457	7	NULL	NULL	0	NULL	Familial mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Familial mutations of the transcription factor RUNX1 ( AML1 , CBFA2 ) predispose to acute myeloid leukemia .
	manualset3
229658	2	421457	7	NULL	NULL	0	NULL	transcription factor	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Familial mutations of the transcription factor RUNX1 ( AML1 , CBFA2 ) predispose to acute myeloid leukemia .
	manualset3
229659	3	421457	7	NULL	NULL	0	NULL	RUNX1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Familial mutations of the transcription factor RUNX1 ( AML1 , CBFA2 ) predispose to acute myeloid leukemia .
	manualset3
229660	4	421457	7	NULL	NULL	0	NULL	AML1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Familial mutations of the transcription factor RUNX1 ( AML1 , CBFA2 ) predispose to acute myeloid leukemia .
	manualset3
229661	5	421457	7	NULL	NULL	0	NULL	CBFA2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Familial mutations of the transcription factor RUNX1 ( AML1 , CBFA2 ) predispose to acute myeloid leukemia .
	manualset3
229662	6	421457	7	NULL	NULL	0	NULL	acute myeloid leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Familial mutations of the transcription factor RUNX1 ( AML1 , CBFA2 ) predispose to acute myeloid leukemia .
	manualset3
229663	1	421458	7	NULL	NULL	0	NULL	Treatments	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatments with phorbol 12-myristate 13-acetate ( PMA ) , a protein kinase C ( PKC ) activator , mimicked the action of thrombin .
	manualset3
229664	2	421458	7	NULL	NULL	0	NULL	phorbol 12-myristate 13-acetate ( PMA )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatments with phorbol 12-myristate 13-acetate ( PMA ) , a protein kinase C ( PKC ) activator , mimicked the action of thrombin .
	manualset3
229665	3	421458	7	NULL	NULL	0	NULL	protein kinase C ( PKC ) activator 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatments with phorbol 12-myristate 13-acetate ( PMA ) , a protein kinase C ( PKC ) activator , mimicked the action of thrombin .
	manualset3
229666	4	421458	7	NULL	NULL	0	NULL	action 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatments with phorbol 12-myristate 13-acetate ( PMA ) , a protein kinase C ( PKC ) activator , mimicked the action of thrombin .
	manualset3
229667	5	421458	7	NULL	NULL	0	NULL	 thrombin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatments with phorbol 12-myristate 13-acetate ( PMA ) , a protein kinase C ( PKC ) activator , mimicked the action of thrombin .
	manualset3
229668	1	421459	7	NULL	NULL	0	NULL	Two groups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two groups of Wistar rats ( G1 and G2 ) were inoculated with 10 ( 4 ) bradyzoites of BTU10 strain ( genotype I ) , p.o. , and other two groups ( G3 and G4 ) were inoculated with 0.9 % saline solution .
	manualset3
229669	2	421459	7	NULL	NULL	0	NULL	Wistar rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two groups of Wistar rats ( G1 and G2 ) were inoculated with 10 ( 4 ) bradyzoites of BTU10 strain ( genotype I ) , p.o. , and other two groups ( G3 and G4 ) were inoculated with 0.9 % saline solution .
	manualset3
229670	3	421459	7	NULL	NULL	0	NULL	G1	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two groups of Wistar rats ( G1 and G2 ) were inoculated with 10 ( 4 ) bradyzoites of BTU10 strain ( genotype I ) , p.o. , and other two groups ( G3 and G4 ) were inoculated with 0.9 % saline solution .
	manualset3
229671	4	421459	7	NULL	NULL	0	NULL	G2	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two groups of Wistar rats ( G1 and G2 ) were inoculated with 10 ( 4 ) bradyzoites of BTU10 strain ( genotype I ) , p.o. , and other two groups ( G3 and G4 ) were inoculated with 0.9 % saline solution .
	manualset3
229672	5	421459	7	NULL	NULL	0	NULL	 10 ( 4 ) bradyzoites	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Two groups of Wistar rats ( G1 and G2 ) were inoculated with 10 ( 4 ) bradyzoites of BTU10 strain ( genotype I ) , p.o. , and other two groups ( G3 and G4 ) were inoculated with 0.9 % saline solution .
	manualset3
229673	6	421459	7	NULL	NULL	0	NULL	BTU10 strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two groups of Wistar rats ( G1 and G2 ) were inoculated with 10 ( 4 ) bradyzoites of BTU10 strain ( genotype I ) , p.o. , and other two groups ( G3 and G4 ) were inoculated with 0.9 % saline solution .
	manualset3
229674	7	421459	7	NULL	NULL	0	NULL	genotype I	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two groups of Wistar rats ( G1 and G2 ) were inoculated with 10 ( 4 ) bradyzoites of BTU10 strain ( genotype I ) , p.o. , and other two groups ( G3 and G4 ) were inoculated with 0.9 % saline solution .
	manualset3
229675	8	421459	7	NULL	NULL	0	NULL	 p.o.	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two groups of Wistar rats ( G1 and G2 ) were inoculated with 10 ( 4 ) bradyzoites of BTU10 strain ( genotype I ) , p.o. , and other two groups ( G3 and G4 ) were inoculated with 0.9 % saline solution .
	manualset3
229676	9	421459	7	NULL	NULL	0	NULL	two groups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two groups of Wistar rats ( G1 and G2 ) were inoculated with 10 ( 4 ) bradyzoites of BTU10 strain ( genotype I ) , p.o. , and other two groups ( G3 and G4 ) were inoculated with 0.9 % saline solution .
	manualset3
229677	10	421459	7	NULL	NULL	0	NULL	G3 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two groups of Wistar rats ( G1 and G2 ) were inoculated with 10 ( 4 ) bradyzoites of BTU10 strain ( genotype I ) , p.o. , and other two groups ( G3 and G4 ) were inoculated with 0.9 % saline solution .
	manualset3
229678	11	421459	7	NULL	NULL	0	NULL	G4	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two groups of Wistar rats ( G1 and G2 ) were inoculated with 10 ( 4 ) bradyzoites of BTU10 strain ( genotype I ) , p.o. , and other two groups ( G3 and G4 ) were inoculated with 0.9 % saline solution .
	manualset3
229679	12	421459	7	NULL	NULL	0	NULL	0.9 % saline solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two groups of Wistar rats ( G1 and G2 ) were inoculated with 10 ( 4 ) bradyzoites of BTU10 strain ( genotype I ) , p.o. , and other two groups ( G3 and G4 ) were inoculated with 0.9 % saline solution .
	manualset3
229680	1	421460	7	NULL	NULL	0	NULL	48	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 48 commercially available PEO-PPO-PEO triblock copolymers , three were selected due to their transparency in the operable range of viscosity and PEO ( 137 ) PPO ( 43 ) PEO ( 137 ) exhibited the most effective separation .
	manualset3
229681	2	421460	7	NULL	NULL	0	NULL	PEO-PPO-PEO triblock copolymers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 48 commercially available PEO-PPO-PEO triblock copolymers , three were selected due to their transparency in the operable range of viscosity and PEO ( 137 ) PPO ( 43 ) PEO ( 137 ) exhibited the most effective separation .
	manualset3
229682	3	421460	7	NULL	NULL	0	NULL	 three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 48 commercially available PEO-PPO-PEO triblock copolymers , three were selected due to their transparency in the operable range of viscosity and PEO ( 137 ) PPO ( 43 ) PEO ( 137 ) exhibited the most effective separation .
	manualset3
229683	4	421460	7	NULL	NULL	0	NULL	operable range	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 48 commercially available PEO-PPO-PEO triblock copolymers , three were selected due to their transparency in the operable range of viscosity and PEO ( 137 ) PPO ( 43 ) PEO ( 137 ) exhibited the most effective separation .
	manualset3
229684	5	421460	7	NULL	NULL	0	NULL	 viscosity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 48 commercially available PEO-PPO-PEO triblock copolymers , three were selected due to their transparency in the operable range of viscosity and PEO ( 137 ) PPO ( 43 ) PEO ( 137 ) exhibited the most effective separation .
	manualset3
229685	6	421460	7	NULL	NULL	0	NULL	PEO ( 137 ) PPO ( 43 ) PEO ( 137 ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 48 commercially available PEO-PPO-PEO triblock copolymers , three were selected due to their transparency in the operable range of viscosity and PEO ( 137 ) PPO ( 43 ) PEO ( 137 ) exhibited the most effective separation .
	manualset3
229686	7	421460	7	NULL	NULL	0	NULL	 effective separation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among 48 commercially available PEO-PPO-PEO triblock copolymers , three were selected due to their transparency in the operable range of viscosity and PEO ( 137 ) PPO ( 43 ) PEO ( 137 ) exhibited the most effective separation .
	manualset3
229687	1	421461	7	NULL	NULL	0	NULL	Two subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two subjects with virologic failure had a population tropism change from CCR5 - to dual/mixed-tropic during treatment .
	manualset3
229688	2	421461	7	NULL	NULL	0	NULL	virologic failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two subjects with virologic failure had a population tropism change from CCR5 - to dual/mixed-tropic during treatment .
	manualset3
229689	3	421461	7	NULL	NULL	0	NULL	population tropism change 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two subjects with virologic failure had a population tropism change from CCR5 - to dual/mixed-tropic during treatment .
	manualset3
229690	4	421461	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Two subjects with virologic failure had a population tropism change from CCR5 - to dual/mixed-tropic during treatment .
	manualset3
231509	5	421461	7	NULL	NULL	0	NULL	CCR5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Two subjects with virologic failure had a population tropism change from CCR5 - to dual/mixed-tropic during treatment .
	manualset3
229691	1	421462	7	NULL	NULL	0	NULL	98 cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional 98 cases were confirmed by non-culture-based methods ( 92 by nucleic acid amplification testing ( NAAT ) and six by serology ) , and where possible serotyping was determined .
	manualset3
229692	2	421462	7	NULL	NULL	0	NULL	non-culture-based methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional 98 cases were confirmed by non-culture-based methods ( 92 by nucleic acid amplification testing ( NAAT ) and six by serology ) , and where possible serotyping was determined .
	manualset3
229693	3	421462	7	NULL	NULL	0	NULL	92 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional 98 cases were confirmed by non-culture-based methods ( 92 by nucleic acid amplification testing ( NAAT ) and six by serology ) , and where possible serotyping was determined .
	manualset3
229694	4	421462	7	NULL	NULL	0	NULL	nucleic acid amplification testing ( NAAT )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional 98 cases were confirmed by non-culture-based methods ( 92 by nucleic acid amplification testing ( NAAT ) and six by serology ) , and where possible serotyping was determined .
	manualset3
229695	5	421462	7	NULL	NULL	0	NULL	 six	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional 98 cases were confirmed by non-culture-based methods ( 92 by nucleic acid amplification testing ( NAAT ) and six by serology ) , and where possible serotyping was determined .
	manualset3
229696	6	421462	7	NULL	NULL	0	NULL	serology 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional 98 cases were confirmed by non-culture-based methods ( 92 by nucleic acid amplification testing ( NAAT ) and six by serology ) , and where possible serotyping was determined .
	manualset3
229697	7	421462	7	NULL	NULL	0	NULL	serotyping 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional 98 cases were confirmed by non-culture-based methods ( 92 by nucleic acid amplification testing ( NAAT ) and six by serology ) , and where possible serotyping was determined .
	manualset3
229698	1	421463	7	NULL	NULL	0	NULL	Sleep continuity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep continuity and architecture : associations with pain-inhibitory processes in patients with temporomandibular joint disorder .
	manualset3
229699	2	421463	7	NULL	NULL	0	NULL	architecture	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep continuity and architecture : associations with pain-inhibitory processes in patients with temporomandibular joint disorder .
	manualset3
229700	3	421463	7	NULL	NULL	0	NULL	associations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep continuity and architecture : associations with pain-inhibitory processes in patients with temporomandibular joint disorder .
	manualset3
229701	4	421463	7	NULL	NULL	0	NULL	pain-inhibitory processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep continuity and architecture : associations with pain-inhibitory processes in patients with temporomandibular joint disorder .
	manualset3
229702	5	421463	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep continuity and architecture : associations with pain-inhibitory processes in patients with temporomandibular joint disorder .
	manualset3
229703	6	421463	7	NULL	NULL	0	NULL	temporomandibular joint disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Sleep continuity and architecture : associations with pain-inhibitory processes in patients with temporomandibular joint disorder .
	manualset3
229704	1	421464	7	NULL	NULL	0	NULL	Conjugated norepinephrine	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Conjugated norepinephrine was also present in plasma of all species except in unstressed rats with access to food .
	manualset3
229705	2	421464	7	NULL	NULL	0	NULL	plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Conjugated norepinephrine was also present in plasma of all species except in unstressed rats with access to food .
	manualset3
229706	3	421464	7	NULL	NULL	0	NULL	species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Conjugated norepinephrine was also present in plasma of all species except in unstressed rats with access to food .
	manualset3
229707	4	421464	7	NULL	NULL	0	NULL	 unstressed rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Conjugated norepinephrine was also present in plasma of all species except in unstressed rats with access to food .
	manualset3
229708	5	421464	7	NULL	NULL	0	NULL	food	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Conjugated norepinephrine was also present in plasma of all species except in unstressed rats with access to food .
	manualset3
229709	1	421465	7	NULL	NULL	0	NULL	Recombinant human bone morphogenetic proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant human bone morphogenetic proteins require the presence of progenitor cells to function .
	manualset3
229710	2	421465	7	NULL	NULL	0	NULL	 presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant human bone morphogenetic proteins require the presence of progenitor cells to function .
	manualset3
229711	3	421465	7	NULL	NULL	0	NULL	progenitor cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant human bone morphogenetic proteins require the presence of progenitor cells to function .
	manualset3
229712	4	421465	7	NULL	NULL	0	NULL	function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recombinant human bone morphogenetic proteins require the presence of progenitor cells to function .
	manualset3
229713	1	421466	7	NULL	NULL	0	NULL	Acne	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Acne , dairy and cancer : The 5alpha-P link .
	manualset3
229714	2	421466	7	NULL	NULL	0	NULL	 dairy 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Acne , dairy and cancer : The 5alpha-P link .
	manualset3
229715	3	421466	7	NULL	NULL	0	NULL	 cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Acne , dairy and cancer : The 5alpha-P link .
	manualset3
229716	4	421466	7	NULL	NULL	0	NULL	5alpha-P link	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Acne , dairy and cancer : The 5alpha-P link .
	manualset3
229717	1	421467	7	NULL	NULL	0	NULL	134 cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 134 cases ( 10.9 % ) transient improvement was observed and only in 50 cases ( 3.8 % ) was BP treatment found to be ineffective .
	manualset3
229718	2	421467	7	NULL	NULL	0	NULL	10.9 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 134 cases ( 10.9 % ) transient improvement was observed and only in 50 cases ( 3.8 % ) was BP treatment found to be ineffective .
	manualset3
229719	3	421467	7	NULL	NULL	0	NULL	transient improvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In 134 cases ( 10.9 % ) transient improvement was observed and only in 50 cases ( 3.8 % ) was BP treatment found to be ineffective .
	manualset3
229720	4	421467	7	NULL	NULL	0	NULL	50 cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 134 cases ( 10.9 % ) transient improvement was observed and only in 50 cases ( 3.8 % ) was BP treatment found to be ineffective .
	manualset3
229721	5	421467	7	NULL	NULL	0	NULL	 3.8 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 134 cases ( 10.9 % ) transient improvement was observed and only in 50 cases ( 3.8 % ) was BP treatment found to be ineffective .
	manualset3
229722	6	421467	7	NULL	NULL	0	NULL	BP treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 134 cases ( 10.9 % ) transient improvement was observed and only in 50 cases ( 3.8 % ) was BP treatment found to be ineffective .
	manualset3
229723	1	421468	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	From these results it can be concluded that a bradykinin B2 receptor is involved in this response .
	manualset3
229724	2	421468	7	NULL	NULL	0	NULL	bradykinin B2 receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	From these results it can be concluded that a bradykinin B2 receptor is involved in this response .
	manualset3
229725	3	421468	7	NULL	NULL	0	NULL	 response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	From these results it can be concluded that a bradykinin B2 receptor is involved in this response .
	manualset3
229726	1	421469	7	NULL	NULL	0	NULL	32	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In 32 of the patients with endocarditis and 35 of those with bacteremia strains were classified as tolerant ( minimum bactericidal concentration/minimum inhibitory concentration greater than or equal to 16 ) .
	manualset3
229727	2	421469	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 32 of the patients with endocarditis and 35 of those with bacteremia strains were classified as tolerant ( minimum bactericidal concentration/minimum inhibitory concentration greater than or equal to 16 ) .
	manualset3
229728	3	421469	7	NULL	NULL	0	NULL	endocarditis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In 32 of the patients with endocarditis and 35 of those with bacteremia strains were classified as tolerant ( minimum bactericidal concentration/minimum inhibitory concentration greater than or equal to 16 ) .
	manualset3
229729	4	421469	7	NULL	NULL	0	NULL	35 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In 32 of the patients with endocarditis and 35 of those with bacteremia strains were classified as tolerant ( minimum bactericidal concentration/minimum inhibitory concentration greater than or equal to 16 ) .
	manualset3
229730	5	421469	7	NULL	NULL	0	NULL	bacteremia strains 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In 32 of the patients with endocarditis and 35 of those with bacteremia strains were classified as tolerant ( minimum bactericidal concentration/minimum inhibitory concentration greater than or equal to 16 ) .
	manualset3
229731	6	421469	7	NULL	NULL	0	NULL	tolerant	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 32 of the patients with endocarditis and 35 of those with bacteremia strains were classified as tolerant ( minimum bactericidal concentration/minimum inhibitory concentration greater than or equal to 16 ) .
	manualset3
229732	7	421469	7	NULL	NULL	0	NULL	minimum bactericidal concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 32 of the patients with endocarditis and 35 of those with bacteremia strains were classified as tolerant ( minimum bactericidal concentration/minimum inhibitory concentration greater than or equal to 16 ) .
	manualset3
229733	8	421469	7	NULL	NULL	0	NULL	minimum inhibitory concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 32 of the patients with endocarditis and 35 of those with bacteremia strains were classified as tolerant ( minimum bactericidal concentration/minimum inhibitory concentration greater than or equal to 16 ) .
	manualset3
229734	9	421469	7	NULL	NULL	0	NULL	16 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In 32 of the patients with endocarditis and 35 of those with bacteremia strains were classified as tolerant ( minimum bactericidal concentration/minimum inhibitory concentration greater than or equal to 16 ) .
	manualset3
229735	1	421470	7	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Without therapy with growth factors , the mean time to neutrophil recovery after discontinuation of the offending agent was reported to be 10 + / - 8 days .
	manualset3
229736	2	421470	7	NULL	NULL	0	NULL	growth factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Without therapy with growth factors , the mean time to neutrophil recovery after discontinuation of the offending agent was reported to be 10 + / - 8 days .
	manualset3
229737	3	421470	7	NULL	NULL	0	NULL	 mean time	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Without therapy with growth factors , the mean time to neutrophil recovery after discontinuation of the offending agent was reported to be 10 + / - 8 days .
	manualset3
229738	4	421470	7	NULL	NULL	0	NULL	neutrophil recovery	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Without therapy with growth factors , the mean time to neutrophil recovery after discontinuation of the offending agent was reported to be 10 + / - 8 days .
	manualset3
229739	5	421470	7	NULL	NULL	0	NULL	discontinuation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Without therapy with growth factors , the mean time to neutrophil recovery after discontinuation of the offending agent was reported to be 10 + / - 8 days .
	manualset3
229740	6	421470	7	NULL	NULL	0	NULL	offending agent 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Without therapy with growth factors , the mean time to neutrophil recovery after discontinuation of the offending agent was reported to be 10 + / - 8 days .
	manualset3
229741	7	421470	7	NULL	NULL	0	NULL	10 + / - 8 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Without therapy with growth factors , the mean time to neutrophil recovery after discontinuation of the offending agent was reported to be 10 + / - 8 days .
	manualset3
229742	1	421471	7	NULL	NULL	0	NULL	conclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The following conclusion , are based on this series of 27 patients , all diabetics with end-stage renal failure : All , except one , with both diabetes and nephropathy exhibited retinopathy .
	manualset3
229743	2	421471	7	NULL	NULL	0	NULL	series	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The following conclusion , are based on this series of 27 patients , all diabetics with end-stage renal failure : All , except one , with both diabetes and nephropathy exhibited retinopathy .
	manualset3
229744	3	421471	7	NULL	NULL	0	NULL	27 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The following conclusion , are based on this series of 27 patients , all diabetics with end-stage renal failure : All , except one , with both diabetes and nephropathy exhibited retinopathy .
	manualset3
229745	4	421471	7	NULL	NULL	0	NULL	 diabetics	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The following conclusion , are based on this series of 27 patients , all diabetics with end-stage renal failure : All , except one , with both diabetes and nephropathy exhibited retinopathy .
	manualset3
229746	5	421471	7	NULL	NULL	0	NULL	end-stage renal failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The following conclusion , are based on this series of 27 patients , all diabetics with end-stage renal failure : All , except one , with both diabetes and nephropathy exhibited retinopathy .
	manualset3
229747	6	421471	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The following conclusion , are based on this series of 27 patients , all diabetics with end-stage renal failure : All , except one , with both diabetes and nephropathy exhibited retinopathy .
	manualset3
229748	7	421471	7	NULL	NULL	0	NULL	diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The following conclusion , are based on this series of 27 patients , all diabetics with end-stage renal failure : All , except one , with both diabetes and nephropathy exhibited retinopathy .
	manualset3
229749	8	421471	7	NULL	NULL	0	NULL	nephropathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The following conclusion , are based on this series of 27 patients , all diabetics with end-stage renal failure : All , except one , with both diabetes and nephropathy exhibited retinopathy .
	manualset3
229750	9	421471	7	NULL	NULL	0	NULL	retinopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The following conclusion , are based on this series of 27 patients , all diabetics with end-stage renal failure : All , except one , with both diabetes and nephropathy exhibited retinopathy .
	manualset3
229751	1	421472	7	NULL	NULL	0	NULL	unexpected finding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An unexpected finding was an excess mortality from oesophageal cancer in both groups .
	manualset3
229752	2	421472	7	NULL	NULL	0	NULL	excess mortality 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An unexpected finding was an excess mortality from oesophageal cancer in both groups .
	manualset3
229753	3	421472	7	NULL	NULL	0	NULL	oesophageal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	An unexpected finding was an excess mortality from oesophageal cancer in both groups .
	manualset3
229754	4	421472	7	NULL	NULL	0	NULL	groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	An unexpected finding was an excess mortality from oesophageal cancer in both groups .
	manualset3
229755	1	421473	7	NULL	NULL	0	NULL	advantage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional advantage was that before challenge and after vaccination with strain 19 , the titers to the IHLT rose later and declined earlier than the titers to the CFT .
	manualset3
229756	2	421473	7	NULL	NULL	0	NULL	 challenge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional advantage was that before challenge and after vaccination with strain 19 , the titers to the IHLT rose later and declined earlier than the titers to the CFT .
	manualset3
229757	3	421473	7	NULL	NULL	0	NULL	vaccination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional advantage was that before challenge and after vaccination with strain 19 , the titers to the IHLT rose later and declined earlier than the titers to the CFT .
	manualset3
229758	4	421473	7	NULL	NULL	0	NULL	strain 19	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional advantage was that before challenge and after vaccination with strain 19 , the titers to the IHLT rose later and declined earlier than the titers to the CFT .
	manualset3
229759	5	421473	7	NULL	NULL	0	NULL	titers 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional advantage was that before challenge and after vaccination with strain 19 , the titers to the IHLT rose later and declined earlier than the titers to the CFT .
	manualset3
229760	6	421473	7	NULL	NULL	0	NULL	IHLT	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional advantage was that before challenge and after vaccination with strain 19 , the titers to the IHLT rose later and declined earlier than the titers to the CFT .
	manualset3
229761	7	421473	7	NULL	NULL	0	NULL	titers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional advantage was that before challenge and after vaccination with strain 19 , the titers to the IHLT rose later and declined earlier than the titers to the CFT .
	manualset3
229762	8	421473	7	NULL	NULL	0	NULL	 CFT	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional advantage was that before challenge and after vaccination with strain 19 , the titers to the IHLT rose later and declined earlier than the titers to the CFT .
	manualset3
229763	1	421474	7	NULL	NULL	0	NULL	Novel mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel mutations of PKD1 gene in Chinese patients with autosomal dominant polycystic kidney disease .
	manualset3
229764	2	421474	7	NULL	NULL	0	NULL	PKD1 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel mutations of PKD1 gene in Chinese patients with autosomal dominant polycystic kidney disease .
	manualset3
229765	3	421474	7	NULL	NULL	0	NULL	Chinese patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel mutations of PKD1 gene in Chinese patients with autosomal dominant polycystic kidney disease .
	manualset3
229766	4	421474	7	NULL	NULL	0	NULL	autosomal dominant polycystic kidney disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Novel mutations of PKD1 gene in Chinese patients with autosomal dominant polycystic kidney disease .
	manualset3
229767	1	421475	7	NULL	NULL	0	NULL	purpose	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this report is to alert clinicians to a possible association between SNRI medications and takotsubo cardiomyopathy .
	manualset3
229768	2	421475	7	NULL	NULL	0	NULL	 report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this report is to alert clinicians to a possible association between SNRI medications and takotsubo cardiomyopathy .
	manualset3
229769	3	421475	7	NULL	NULL	0	NULL	clinicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this report is to alert clinicians to a possible association between SNRI medications and takotsubo cardiomyopathy .
	manualset3
229770	4	421475	7	NULL	NULL	0	NULL	association 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this report is to alert clinicians to a possible association between SNRI medications and takotsubo cardiomyopathy .
	manualset3
229771	5	421475	7	NULL	NULL	0	NULL	SNRI medications	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this report is to alert clinicians to a possible association between SNRI medications and takotsubo cardiomyopathy .
	manualset3
229772	6	421475	7	NULL	NULL	0	NULL	takotsubo cardiomyopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of this report is to alert clinicians to a possible association between SNRI medications and takotsubo cardiomyopathy .
	manualset3
229773	1	421476	7	NULL	NULL	0	NULL	mitochondria 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitochondria were apparently the target organelle in Y79 retinoblastoma cells .
	manualset3
229774	2	421476	7	NULL	NULL	0	NULL	target organelle	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitochondria were apparently the target organelle in Y79 retinoblastoma cells .
	manualset3
229775	3	421476	7	NULL	NULL	0	NULL	Y79 retinoblastoma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The mitochondria were apparently the target organelle in Y79 retinoblastoma cells .
	manualset3
229776	1	421477	7	NULL	NULL	0	NULL	Structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure and expression of a cloned cDNA for human ( 2 ' -5 ' ) oligoadenylate synthetase .
	manualset3
229777	2	421477	7	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure and expression of a cloned cDNA for human ( 2 ' -5 ' ) oligoadenylate synthetase .
	manualset3
229778	3	421477	7	NULL	NULL	0	NULL	 cloned cDNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure and expression of a cloned cDNA for human ( 2 ' -5 ' ) oligoadenylate synthetase .
	manualset3
229779	4	421477	7	NULL	NULL	0	NULL	human ( 2 ' -5 ' ) oligoadenylate synthetase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Structure and expression of a cloned cDNA for human ( 2 ' -5 ' ) oligoadenylate synthetase .
	manualset3
229780	1	421478	7	NULL	NULL	0	NULL	recorded differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The recorded differences in spatial distribution and resource use might expose male and female to distinct threats , thus affecting population dynamics through differential mortality .
	manualset3
229781	2	421478	7	NULL	NULL	0	NULL	spatial distribution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The recorded differences in spatial distribution and resource use might expose male and female to distinct threats , thus affecting population dynamics through differential mortality .
	manualset3
229782	3	421478	7	NULL	NULL	0	NULL	resource use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The recorded differences in spatial distribution and resource use might expose male and female to distinct threats , thus affecting population dynamics through differential mortality .
	manualset3
229783	4	421478	7	NULL	NULL	0	NULL	male	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The recorded differences in spatial distribution and resource use might expose male and female to distinct threats , thus affecting population dynamics through differential mortality .
	manualset3
229784	5	421478	7	NULL	NULL	0	NULL	female	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The recorded differences in spatial distribution and resource use might expose male and female to distinct threats , thus affecting population dynamics through differential mortality .
	manualset3
229785	6	421478	7	NULL	NULL	NULL	NULL	population dynamics	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The recorded differences in spatial distribution and resource use might expose male and female to distinct threats , thus affecting population dynamics through differential mortality .
	manualset3
229786	7	421478	7	NULL	NULL	0	NULL	differential mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The recorded differences in spatial distribution and resource use might expose male and female to distinct threats , thus affecting population dynamics through differential mortality .
	manualset3
231608	8	421478	7	NULL	NULL	0	NULL	threats	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The recorded differences in spatial distribution and resource use might expose male and female to distinct threats , thus affecting population dynamics through differential mortality .
	manualset3
229787	1	421479	7	NULL	NULL	0	NULL	additional barrier	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional barrier is the widespread belief among husbands that if women are protected from conceiving , they will engage in extramarital relations .
	manualset3
229788	2	421479	7	NULL	NULL	0	NULL	widespread belief	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional barrier is the widespread belief among husbands that if women are protected from conceiving , they will engage in extramarital relations .
	manualset3
229789	3	421479	7	NULL	NULL	0	NULL	husbands	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional barrier is the widespread belief among husbands that if women are protected from conceiving , they will engage in extramarital relations .
	manualset3
229790	4	421479	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional barrier is the widespread belief among husbands that if women are protected from conceiving , they will engage in extramarital relations .
	manualset3
229791	5	421479	7	NULL	NULL	0	NULL	extramarital relations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional barrier is the widespread belief among husbands that if women are protected from conceiving , they will engage in extramarital relations .
	manualset3
231609	6	421479	7	NULL	NULL	0	NULL	 conceiving	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional barrier is the widespread belief among husbands that if women are protected from conceiving , they will engage in extramarital relations .
	manualset3
229792	1	421480	7	NULL	NULL	0	NULL	comparative study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative study of the degree of severity gives the following percentages of success : mitral stenosis , 85 % ( pulsed Doppler ) vs 71 % ( continuous Doppler ) for mitral stenoses ; aortic stenoses 83 % ( pulsed Doppler ) vs 58 % ( continuous Doppler ) .
	manualset3
229793	2	421480	7	NULL	NULL	0	NULL	degree of severity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative study of the degree of severity gives the following percentages of success : mitral stenosis , 85 % ( pulsed Doppler ) vs 71 % ( continuous Doppler ) for mitral stenoses ; aortic stenoses 83 % ( pulsed Doppler ) vs 58 % ( continuous Doppler ) .
	manualset3
229794	3	421480	7	NULL	NULL	0	NULL	 percentages	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative study of the degree of severity gives the following percentages of success : mitral stenosis , 85 % ( pulsed Doppler ) vs 71 % ( continuous Doppler ) for mitral stenoses ; aortic stenoses 83 % ( pulsed Doppler ) vs 58 % ( continuous Doppler ) .
	manualset3
229795	4	421480	7	NULL	NULL	0	NULL	success	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative study of the degree of severity gives the following percentages of success : mitral stenosis , 85 % ( pulsed Doppler ) vs 71 % ( continuous Doppler ) for mitral stenoses ; aortic stenoses 83 % ( pulsed Doppler ) vs 58 % ( continuous Doppler ) .
	manualset3
229796	5	421480	7	NULL	NULL	0	NULL	mitral stenosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative study of the degree of severity gives the following percentages of success : mitral stenosis , 85 % ( pulsed Doppler ) vs 71 % ( continuous Doppler ) for mitral stenoses ; aortic stenoses 83 % ( pulsed Doppler ) vs 58 % ( continuous Doppler ) .
	manualset3
229797	6	421480	7	NULL	NULL	0	NULL	85 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative study of the degree of severity gives the following percentages of success : mitral stenosis , 85 % ( pulsed Doppler ) vs 71 % ( continuous Doppler ) for mitral stenoses ; aortic stenoses 83 % ( pulsed Doppler ) vs 58 % ( continuous Doppler ) .
	manualset3
229798	7	421480	7	NULL	NULL	0	NULL	pulsed Doppler	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative study of the degree of severity gives the following percentages of success : mitral stenosis , 85 % ( pulsed Doppler ) vs 71 % ( continuous Doppler ) for mitral stenoses ; aortic stenoses 83 % ( pulsed Doppler ) vs 58 % ( continuous Doppler ) .
	manualset3
229799	8	421480	7	NULL	NULL	0	NULL	71 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative study of the degree of severity gives the following percentages of success : mitral stenosis , 85 % ( pulsed Doppler ) vs 71 % ( continuous Doppler ) for mitral stenoses ; aortic stenoses 83 % ( pulsed Doppler ) vs 58 % ( continuous Doppler ) .
	manualset3
229800	9	421480	7	NULL	NULL	0	NULL	continuous Doppler 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative study of the degree of severity gives the following percentages of success : mitral stenosis , 85 % ( pulsed Doppler ) vs 71 % ( continuous Doppler ) for mitral stenoses ; aortic stenoses 83 % ( pulsed Doppler ) vs 58 % ( continuous Doppler ) .
	manualset3
229801	10	421480	7	NULL	NULL	0	NULL	mitral stenoses	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative study of the degree of severity gives the following percentages of success : mitral stenosis , 85 % ( pulsed Doppler ) vs 71 % ( continuous Doppler ) for mitral stenoses ; aortic stenoses 83 % ( pulsed Doppler ) vs 58 % ( continuous Doppler ) .
	manualset3
229802	11	421480	7	NULL	NULL	0	NULL	aortic stenoses	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative study of the degree of severity gives the following percentages of success : mitral stenosis , 85 % ( pulsed Doppler ) vs 71 % ( continuous Doppler ) for mitral stenoses ; aortic stenoses 83 % ( pulsed Doppler ) vs 58 % ( continuous Doppler ) .
	manualset3
229803	12	421480	7	NULL	NULL	0	NULL	83 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative study of the degree of severity gives the following percentages of success : mitral stenosis , 85 % ( pulsed Doppler ) vs 71 % ( continuous Doppler ) for mitral stenoses ; aortic stenoses 83 % ( pulsed Doppler ) vs 58 % ( continuous Doppler ) .
	manualset3
229804	13	421480	7	NULL	NULL	0	NULL	pulsed Doppler	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative study of the degree of severity gives the following percentages of success : mitral stenosis , 85 % ( pulsed Doppler ) vs 71 % ( continuous Doppler ) for mitral stenoses ; aortic stenoses 83 % ( pulsed Doppler ) vs 58 % ( continuous Doppler ) .
	manualset3
229805	14	421480	7	NULL	NULL	0	NULL	58 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative study of the degree of severity gives the following percentages of success : mitral stenosis , 85 % ( pulsed Doppler ) vs 71 % ( continuous Doppler ) for mitral stenoses ; aortic stenoses 83 % ( pulsed Doppler ) vs 58 % ( continuous Doppler ) .
	manualset3
229806	15	421480	7	NULL	NULL	0	NULL	continuous Doppler	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The comparative study of the degree of severity gives the following percentages of success : mitral stenosis , 85 % ( pulsed Doppler ) vs 71 % ( continuous Doppler ) for mitral stenoses ; aortic stenoses 83 % ( pulsed Doppler ) vs 58 % ( continuous Doppler ) .
	manualset3
229807	1	421481	7	NULL	NULL	0	NULL	American Heart Association	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	American Heart Association issues guidelines on imaging in transient ischemic attacks and stroke .
	manualset3
229808	2	421481	7	NULL	NULL	0	NULL	guidelines	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	American Heart Association issues guidelines on imaging in transient ischemic attacks and stroke .
	manualset3
229809	3	421481	7	NULL	NULL	0	NULL	 imaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	American Heart Association issues guidelines on imaging in transient ischemic attacks and stroke .
	manualset3
229810	4	421481	7	NULL	NULL	0	NULL	transient ischemic attacks	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	American Heart Association issues guidelines on imaging in transient ischemic attacks and stroke .
	manualset3
229811	5	421481	7	NULL	NULL	0	NULL	stroke	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	American Heart Association issues guidelines on imaging in transient ischemic attacks and stroke .
	manualset3
229812	1	421482	7	NULL	NULL	0	NULL	scarring	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Some scarring was a common sequel and resulting fear of dogs remained with some children .
	manualset3
229813	2	421482	7	NULL	NULL	0	NULL	common sequel 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Some scarring was a common sequel and resulting fear of dogs remained with some children .
	manualset3
229814	3	421482	7	NULL	NULL	0	NULL	fear	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Some scarring was a common sequel and resulting fear of dogs remained with some children .
	manualset3
229815	4	421482	7	NULL	NULL	0	NULL	 dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Some scarring was a common sequel and resulting fear of dogs remained with some children .
	manualset3
229816	5	421482	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Some scarring was a common sequel and resulting fear of dogs remained with some children .
	manualset3
229817	1	421483	7	NULL	NULL	0	NULL	Biophysical assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Biophysical assays revealed that MaviP35 proteins produced in bacteria and yeast had similar primary and secondary structures .
	manualset3
229818	2	421483	7	NULL	NULL	0	NULL	MaviP35 proteins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Biophysical assays revealed that MaviP35 proteins produced in bacteria and yeast had similar primary and secondary structures .
	manualset3
229819	3	421483	7	NULL	NULL	0	NULL	 bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Biophysical assays revealed that MaviP35 proteins produced in bacteria and yeast had similar primary and secondary structures .
	manualset3
229820	4	421483	7	NULL	NULL	0	NULL	yeast	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Biophysical assays revealed that MaviP35 proteins produced in bacteria and yeast had similar primary and secondary structures .
	manualset3
229821	5	421483	7	NULL	NULL	0	NULL	primary structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Biophysical assays revealed that MaviP35 proteins produced in bacteria and yeast had similar primary and secondary structures .
	manualset3
229822	6	421483	7	NULL	NULL	0	NULL	secondary structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Biophysical assays revealed that MaviP35 proteins produced in bacteria and yeast had similar primary and secondary structures .
	manualset3
229823	1	421484	7	NULL	NULL	0	NULL	inhibitory capacities 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory capacities of six different disintegrins and one related neurotoxin analog for the binding of RGD-dependent integrins to either fibrinogen , vitronectin or fibronectin were compared in solid phase assays .
	manualset3
229824	2	421484	7	NULL	NULL	0	NULL	six different disintegrins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory capacities of six different disintegrins and one related neurotoxin analog for the binding of RGD-dependent integrins to either fibrinogen , vitronectin or fibronectin were compared in solid phase assays .
	manualset3
229825	3	421484	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory capacities of six different disintegrins and one related neurotoxin analog for the binding of RGD-dependent integrins to either fibrinogen , vitronectin or fibronectin were compared in solid phase assays .
	manualset3
229826	4	421484	7	NULL	NULL	NULL	NULL	neurotoxin analog	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The inhibitory capacities of six different disintegrins and one related neurotoxin analog for the binding of RGD-dependent integrins to either fibrinogen , vitronectin or fibronectin were compared in solid phase assays .
	manualset3
229827	5	421484	7	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory capacities of six different disintegrins and one related neurotoxin analog for the binding of RGD-dependent integrins to either fibrinogen , vitronectin or fibronectin were compared in solid phase assays .
	manualset3
229828	6	421484	7	NULL	NULL	0	NULL	RGD-dependent integrins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory capacities of six different disintegrins and one related neurotoxin analog for the binding of RGD-dependent integrins to either fibrinogen , vitronectin or fibronectin were compared in solid phase assays .
	manualset3
229829	7	421484	7	NULL	NULL	0	NULL	fibrinogen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory capacities of six different disintegrins and one related neurotoxin analog for the binding of RGD-dependent integrins to either fibrinogen , vitronectin or fibronectin were compared in solid phase assays .
	manualset3
229830	8	421484	7	NULL	NULL	0	NULL	vitronectin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory capacities of six different disintegrins and one related neurotoxin analog for the binding of RGD-dependent integrins to either fibrinogen , vitronectin or fibronectin were compared in solid phase assays .
	manualset3
229831	9	421484	7	NULL	NULL	0	NULL	fibronectin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory capacities of six different disintegrins and one related neurotoxin analog for the binding of RGD-dependent integrins to either fibrinogen , vitronectin or fibronectin were compared in solid phase assays .
	manualset3
229832	10	421484	7	NULL	NULL	0	NULL	solid phase assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The inhibitory capacities of six different disintegrins and one related neurotoxin analog for the binding of RGD-dependent integrins to either fibrinogen , vitronectin or fibronectin were compared in solid phase assays .
	manualset3
229833	1	421485	7	NULL	NULL	0	NULL	neutrophils	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We found that neutrophils were rapidly recruited to the lungs following i.n. inoculation of the pathogen and declined to baseline level upon clearance of the infection .
	manualset3
229834	2	421485	7	NULL	NULL	0	NULL	 lungs 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We found that neutrophils were rapidly recruited to the lungs following i.n. inoculation of the pathogen and declined to baseline level upon clearance of the infection .
	manualset3
229835	3	421485	7	NULL	NULL	NULL	NULL	 i.n. inoculation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We found that neutrophils were rapidly recruited to the lungs following i.n. inoculation of the pathogen and declined to baseline level upon clearance of the infection .
	manualset3
229836	4	421485	7	NULL	NULL	0	NULL	pathogen	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We found that neutrophils were rapidly recruited to the lungs following i.n. inoculation of the pathogen and declined to baseline level upon clearance of the infection .
	manualset3
229837	5	421485	7	NULL	NULL	0	NULL	baseline level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We found that neutrophils were rapidly recruited to the lungs following i.n. inoculation of the pathogen and declined to baseline level upon clearance of the infection .
	manualset3
229838	6	421485	7	NULL	NULL	0	NULL	clearance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We found that neutrophils were rapidly recruited to the lungs following i.n. inoculation of the pathogen and declined to baseline level upon clearance of the infection .
	manualset3
229839	7	421485	7	NULL	NULL	0	NULL	 infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We found that neutrophils were rapidly recruited to the lungs following i.n. inoculation of the pathogen and declined to baseline level upon clearance of the infection .
	manualset3
229840	1	421486	7	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The number and mitotic activity of the germinal cells in the follicle bulb were determined after administration of colchicine .
	manualset3
229841	2	421486	7	NULL	NULL	0	NULL	mitotic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The number and mitotic activity of the germinal cells in the follicle bulb were determined after administration of colchicine .
	manualset3
229842	3	421486	7	NULL	NULL	0	NULL	germinal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The number and mitotic activity of the germinal cells in the follicle bulb were determined after administration of colchicine .
	manualset3
229843	4	421486	7	NULL	NULL	0	NULL	follicle bulb	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The number and mitotic activity of the germinal cells in the follicle bulb were determined after administration of colchicine .
	manualset3
229844	5	421486	7	NULL	NULL	0	NULL	administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The number and mitotic activity of the germinal cells in the follicle bulb were determined after administration of colchicine .
	manualset3
229845	6	421486	7	NULL	NULL	0	NULL	colchicine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The number and mitotic activity of the germinal cells in the follicle bulb were determined after administration of colchicine .
	manualset3
229846	1	421487	7	NULL	NULL	0	NULL	additional benefit 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional benefit will be a gain of about 500 million years of life over the 10 years from 2006 to 2015 .
	manualset3
229847	2	421487	7	NULL	NULL	0	NULL	gain 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional benefit will be a gain of about 500 million years of life over the 10 years from 2006 to 2015 .
	manualset3
229848	3	421487	7	NULL	NULL	0	NULL	500 million years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional benefit will be a gain of about 500 million years of life over the 10 years from 2006 to 2015 .
	manualset3
229849	4	421487	7	NULL	NULL	0	NULL	 life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional benefit will be a gain of about 500 million years of life over the 10 years from 2006 to 2015 .
	manualset3
229850	5	421487	7	NULL	NULL	0	NULL	10 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional benefit will be a gain of about 500 million years of life over the 10 years from 2006 to 2015 .
	manualset3
229851	6	421487	7	NULL	NULL	0	NULL	2006 to 2015	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional benefit will be a gain of about 500 million years of life over the 10 years from 2006 to 2015 .
	manualset3
229852	1	421488	7	NULL	NULL	0	NULL	 improved sensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the improved sensitivity and specificity achieved , the ILO Classification also allows comparison with other studies .
	manualset3
229853	2	421488	7	NULL	NULL	0	NULL	specificity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the improved sensitivity and specificity achieved , the ILO Classification also allows comparison with other studies .
	manualset3
229854	3	421488	7	NULL	NULL	0	NULL	 ILO Classification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the improved sensitivity and specificity achieved , the ILO Classification also allows comparison with other studies .
	manualset3
229855	4	421488	7	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the improved sensitivity and specificity achieved , the ILO Classification also allows comparison with other studies .
	manualset3
229856	5	421488	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to the improved sensitivity and specificity achieved , the ILO Classification also allows comparison with other studies .
	manualset3
229857	1	421489	7	NULL	NULL	0	NULL	analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	These analyses revealed that PPR531-11 has a role in intergenic RNA cleavage between clpP and 5 ' - rps12 and in the splicing of clpP pre-mRNA .
	manualset3
229858	2	421489	7	NULL	NULL	0	NULL	PPR531-11	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These analyses revealed that PPR531-11 has a role in intergenic RNA cleavage between clpP and 5 ' - rps12 and in the splicing of clpP pre-mRNA .
	manualset3
229859	3	421489	7	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These analyses revealed that PPR531-11 has a role in intergenic RNA cleavage between clpP and 5 ' - rps12 and in the splicing of clpP pre-mRNA .
	manualset3
229860	4	421489	7	NULL	NULL	0	NULL	 intergenic RNA cleavage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These analyses revealed that PPR531-11 has a role in intergenic RNA cleavage between clpP and 5 ' - rps12 and in the splicing of clpP pre-mRNA .
	manualset3
229861	5	421489	7	NULL	NULL	0	NULL	clpP	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	These analyses revealed that PPR531-11 has a role in intergenic RNA cleavage between clpP and 5 ' - rps12 and in the splicing of clpP pre-mRNA .
	manualset3
229862	6	421489	7	NULL	NULL	0	NULL	 5 ' - rps12	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	These analyses revealed that PPR531-11 has a role in intergenic RNA cleavage between clpP and 5 ' - rps12 and in the splicing of clpP pre-mRNA .
	manualset3
229863	7	421489	7	NULL	NULL	0	NULL	splicing	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These analyses revealed that PPR531-11 has a role in intergenic RNA cleavage between clpP and 5 ' - rps12 and in the splicing of clpP pre-mRNA .
	manualset3
229864	8	421489	7	NULL	NULL	0	NULL	clpP pre-mRNA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	These analyses revealed that PPR531-11 has a role in intergenic RNA cleavage between clpP and 5 ' - rps12 and in the splicing of clpP pre-mRNA .
	manualset3
229865	1	421490	7	NULL	NULL	0	NULL	Purification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Purification and properties of pyridoxal phosphate phosphatase .
	manualset3
229866	2	421490	7	NULL	NULL	0	NULL	properties	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Purification and properties of pyridoxal phosphate phosphatase .
	manualset3
229867	3	421490	7	NULL	NULL	0	NULL	 pyridoxal phosphate phosphatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Purification and properties of pyridoxal phosphate phosphatase .
	manualset3
229868	1	421491	7	NULL	NULL	0	NULL	Vibrational spectroscopic , first-order hyperpolarizability	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Vibrational spectroscopic , first-order hyperpolarizability and HOMO , LUMO studies of 4-chloro-2 - ( trifluoromethyl ) aniline based on DFT calculations .
	manualset3
229869	2	421491	7	NULL	NULL	0	NULL	HOMO	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Vibrational spectroscopic , first-order hyperpolarizability and HOMO , LUMO studies of 4-chloro-2 - ( trifluoromethyl ) aniline based on DFT calculations .
	manualset3
229870	3	421491	7	NULL	NULL	0	NULL	LUMO studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Vibrational spectroscopic , first-order hyperpolarizability and HOMO , LUMO studies of 4-chloro-2 - ( trifluoromethyl ) aniline based on DFT calculations .
	manualset3
229871	4	421491	7	NULL	NULL	NULL	NULL	4-chloro-2 - ( trifluoromethyl ) aniline	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Vibrational spectroscopic , first-order hyperpolarizability and HOMO , LUMO studies of 4-chloro-2 - ( trifluoromethyl ) aniline based on DFT calculations .
	manualset3
229872	5	421491	7	NULL	NULL	0	NULL	DFT calculations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Vibrational spectroscopic , first-order hyperpolarizability and HOMO , LUMO studies of 4-chloro-2 - ( trifluoromethyl ) aniline based on DFT calculations .
	manualset3
229873	1	421492	7	NULL	NULL	0	NULL	Criteria	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Criteria for the diagnosis of adenomyosis vary widely in practice .
	manualset3
229874	2	421492	7	NULL	NULL	0	NULL	diagnosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Criteria for the diagnosis of adenomyosis vary widely in practice .
	manualset3
229875	3	421492	7	NULL	NULL	0	NULL	adenomyosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Criteria for the diagnosis of adenomyosis vary widely in practice .
	manualset3
229876	4	421492	7	NULL	NULL	0	NULL	practice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Criteria for the diagnosis of adenomyosis vary widely in practice .
	manualset3
230014	1	421493	7	NULL	NULL	0	NULL	TOM-network N	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	For a TOM-network N , suppose that the set X consisting of the leaves and the root is known , together with the distances between members of X. It is proved that N is uniquely determined from this information and can be reconstructed in polynomial time .
	manualset3
230015	2	421493	7	NULL	NULL	0	NULL	set X 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	For a TOM-network N , suppose that the set X consisting of the leaves and the root is known , together with the distances between members of X. It is proved that N is uniquely determined from this information and can be reconstructed in polynomial time .
	manualset3
230016	3	421493	7	NULL	NULL	0	NULL	leaves 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	For a TOM-network N , suppose that the set X consisting of the leaves and the root is known , together with the distances between members of X. It is proved that N is uniquely determined from this information and can be reconstructed in polynomial time .
	manualset3
230017	4	421493	7	NULL	NULL	0	NULL	root 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	For a TOM-network N , suppose that the set X consisting of the leaves and the root is known , together with the distances between members of X. It is proved that N is uniquely determined from this information and can be reconstructed in polynomial time .
	manualset3
230018	5	421493	7	NULL	NULL	0	NULL	distances	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For a TOM-network N , suppose that the set X consisting of the leaves and the root is known , together with the distances between members of X. It is proved that N is uniquely determined from this information and can be reconstructed in polynomial time .
	manualset3
230019	6	421493	7	NULL	NULL	0	NULL	members	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	For a TOM-network N , suppose that the set X consisting of the leaves and the root is known , together with the distances between members of X. It is proved that N is uniquely determined from this information and can be reconstructed in polynomial time .
	manualset3
230020	7	421493	7	NULL	NULL	0	NULL	 X	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	For a TOM-network N , suppose that the set X consisting of the leaves and the root is known , together with the distances between members of X. It is proved that N is uniquely determined from this information and can be reconstructed in polynomial time .
	manualset3
230021	8	421493	7	NULL	NULL	0	NULL	N	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	For a TOM-network N , suppose that the set X consisting of the leaves and the root is known , together with the distances between members of X. It is proved that N is uniquely determined from this information and can be reconstructed in polynomial time .
	manualset3
230022	9	421493	7	NULL	NULL	0	NULL	 information 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	For a TOM-network N , suppose that the set X consisting of the leaves and the root is known , together with the distances between members of X. It is proved that N is uniquely determined from this information and can be reconstructed in polynomial time .
	manualset3
230023	10	421493	7	NULL	NULL	0	NULL	polynomial time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	For a TOM-network N , suppose that the set X consisting of the leaves and the root is known , together with the distances between members of X. It is proved that N is uniquely determined from this information and can be reconstructed in polynomial time .
	manualset3
230024	1	421494	7	NULL	NULL	0	NULL	concern	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional concern is the potential of P. gigantea to acquire a necrotrophic habit through adaptation to living wood tissues .
	manualset3
230025	2	421494	7	NULL	NULL	0	NULL	potential	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional concern is the potential of P. gigantea to acquire a necrotrophic habit through adaptation to living wood tissues .
	manualset3
230026	3	421494	7	NULL	NULL	0	NULL	P. gigantea 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional concern is the potential of P. gigantea to acquire a necrotrophic habit through adaptation to living wood tissues .
	manualset3
230027	4	421494	7	NULL	NULL	0	NULL	necrotrophic habit 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional concern is the potential of P. gigantea to acquire a necrotrophic habit through adaptation to living wood tissues .
	manualset3
230029	5	421494	7	NULL	NULL	0	NULL	adaptation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional concern is the potential of P. gigantea to acquire a necrotrophic habit through adaptation to living wood tissues .
	manualset3
230032	6	421494	7	NULL	NULL	0	NULL	living wood tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional concern is the potential of P. gigantea to acquire a necrotrophic habit through adaptation to living wood tissues .
	manualset3
230045	1	421495	7	NULL	NULL	0	NULL	maternal provisioning	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The maternal provisioning of yolk to eggs transfers significant quantities of persistent organic pollutants ( POPs ) .
	manualset3
230046	2	421495	7	NULL	NULL	NULL	NULL	yolk	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The maternal provisioning of yolk to eggs transfers significant quantities of persistent organic pollutants ( POPs ) .
	manualset3
230047	3	421495	7	NULL	NULL	NULL	NULL	eggs 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The maternal provisioning of yolk to eggs transfers significant quantities of persistent organic pollutants ( POPs ) .
	manualset3
230050	4	421495	7	NULL	NULL	0	NULL	quantities	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The maternal provisioning of yolk to eggs transfers significant quantities of persistent organic pollutants ( POPs ) .
	manualset3
230052	5	421495	7	NULL	NULL	0	NULL	persistent organic pollutants ( POPs )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The maternal provisioning of yolk to eggs transfers significant quantities of persistent organic pollutants ( POPs ) .
	manualset3
230071	1	421496	7	NULL	NULL	0	NULL	Biosynthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Biosynthesis of acyl dihydroxyacetone phosphate in subcellular fractions of rat liver .
	manualset3
230073	2	421496	7	NULL	NULL	0	NULL	acyl dihydroxyacetone phosphate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Biosynthesis of acyl dihydroxyacetone phosphate in subcellular fractions of rat liver .
	manualset3
230076	3	421496	7	NULL	NULL	0	NULL	subcellular fractions	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Biosynthesis of acyl dihydroxyacetone phosphate in subcellular fractions of rat liver .
	manualset3
230079	4	421496	7	NULL	NULL	0	NULL	rat liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Biosynthesis of acyl dihydroxyacetone phosphate in subcellular fractions of rat liver .
	manualset3
230094	1	421497	7	NULL	NULL	0	NULL	Asymptotic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Asymptotic analysis of stresses near a crack tip in a two-dimensional colloidal packing saturated with liquid .
	manualset3
230095	2	421497	7	NULL	NULL	0	NULL	stresses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Asymptotic analysis of stresses near a crack tip in a two-dimensional colloidal packing saturated with liquid .
	manualset3
230096	3	421497	7	NULL	NULL	0	NULL	crack tip	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Asymptotic analysis of stresses near a crack tip in a two-dimensional colloidal packing saturated with liquid .
	manualset3
230097	4	421497	7	NULL	NULL	0	NULL	two-dimensional colloidal packing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Asymptotic analysis of stresses near a crack tip in a two-dimensional colloidal packing saturated with liquid .
	manualset3
230098	5	421497	7	NULL	NULL	0	NULL	 liquid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Asymptotic analysis of stresses near a crack tip in a two-dimensional colloidal packing saturated with liquid .
	manualset3
230099	1	421498	7	NULL	NULL	NULL	NULL	aspects	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Although these aspects of polyprotein processing are well characterized , the function of 2A is unknown .
	manualset3
230100	2	421498	7	NULL	NULL	0	NULL	polyprotein processing	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these aspects of polyprotein processing are well characterized , the function of 2A is unknown .
	manualset3
230101	3	421498	7	NULL	NULL	0	NULL	function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these aspects of polyprotein processing are well characterized , the function of 2A is unknown .
	manualset3
230102	4	421498	7	NULL	NULL	0	NULL	2A	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although these aspects of polyprotein processing are well characterized , the function of 2A is unknown .
	manualset3
230103	1	421499	7	NULL	NULL	0	NULL	 first two groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The first two groups comprised 17 patients with resistant constipation , with or without megacolon or dolichocolon .
	manualset3
230104	2	421499	7	NULL	NULL	0	NULL	17 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The first two groups comprised 17 patients with resistant constipation , with or without megacolon or dolichocolon .
	manualset3
230105	3	421499	7	NULL	NULL	0	NULL	resistant constipation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The first two groups comprised 17 patients with resistant constipation , with or without megacolon or dolichocolon .
	manualset3
230106	4	421499	7	NULL	NULL	0	NULL	megacolon 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The first two groups comprised 17 patients with resistant constipation , with or without megacolon or dolichocolon .
	manualset3
230107	5	421499	7	NULL	NULL	0	NULL	dolichocolon 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The first two groups comprised 17 patients with resistant constipation , with or without megacolon or dolichocolon .
	manualset3
230108	1	421500	7	NULL	NULL	0	NULL	 therapeutic agent	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Determining the exact `` therapeutic agent '' in IVIG for each specific disease state may allow for a more tailored approach to treatment ( i.e. , isolation or production of the particular antibody ) .
	manualset3
230109	2	421500	7	NULL	NULL	0	NULL	IVIG	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Determining the exact `` therapeutic agent '' in IVIG for each specific disease state may allow for a more tailored approach to treatment ( i.e. , isolation or production of the particular antibody ) .
	manualset3
230110	3	421500	7	NULL	NULL	0	NULL	disease state	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Determining the exact `` therapeutic agent '' in IVIG for each specific disease state may allow for a more tailored approach to treatment ( i.e. , isolation or production of the particular antibody ) .
	manualset3
230111	4	421500	7	NULL	NULL	0	NULL	tailored approach 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Determining the exact `` therapeutic agent '' in IVIG for each specific disease state may allow for a more tailored approach to treatment ( i.e. , isolation or production of the particular antibody ) .
	manualset3
230112	5	421500	7	NULL	NULL	0	NULL	 treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Determining the exact `` therapeutic agent '' in IVIG for each specific disease state may allow for a more tailored approach to treatment ( i.e. , isolation or production of the particular antibody ) .
	manualset3
230113	6	421500	7	NULL	NULL	0	NULL	isolation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Determining the exact `` therapeutic agent '' in IVIG for each specific disease state may allow for a more tailored approach to treatment ( i.e. , isolation or production of the particular antibody ) .
	manualset3
230114	7	421500	7	NULL	NULL	0	NULL	production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Determining the exact `` therapeutic agent '' in IVIG for each specific disease state may allow for a more tailored approach to treatment ( i.e. , isolation or production of the particular antibody ) .
	manualset3
230115	8	421500	7	NULL	NULL	0	NULL	antibody 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Determining the exact `` therapeutic agent '' in IVIG for each specific disease state may allow for a more tailored approach to treatment ( i.e. , isolation or production of the particular antibody ) .
	manualset3
230116	1	421501	7	NULL	NULL	0	NULL	 financing source	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional financing source such as CMI may substantially improve the state of surgical clinics , provided that optimal conditions for surgeons ' work were created .
	manualset3
230117	2	421501	7	NULL	NULL	0	NULL	CMI	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional financing source such as CMI may substantially improve the state of surgical clinics , provided that optimal conditions for surgeons ' work were created .
	manualset3
230118	3	421501	7	NULL	NULL	0	NULL	state 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional financing source such as CMI may substantially improve the state of surgical clinics , provided that optimal conditions for surgeons ' work were created .
	manualset3
230119	4	421501	7	NULL	NULL	0	NULL	surgical clinics	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional financing source such as CMI may substantially improve the state of surgical clinics , provided that optimal conditions for surgeons ' work were created .
	manualset3
230120	5	421501	7	NULL	NULL	0	NULL	optimal conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional financing source such as CMI may substantially improve the state of surgical clinics , provided that optimal conditions for surgeons ' work were created .
	manualset3
230121	6	421501	7	NULL	NULL	0	NULL	surgeons ' work 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional financing source such as CMI may substantially improve the state of surgical clinics , provided that optimal conditions for surgeons ' work were created .
	manualset3
230186	1	421502	7	NULL	NULL	0	NULL	perfluorochemical oxygen-transport fluid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We gave a perfluorochemical oxygen-transport fluid and plasma expander , Fluosol-DA , to seven severely anemic patients before surgery to determine its effectiveness in supplementing oxygen transport .
	manualset3
230187	2	421502	7	NULL	NULL	0	NULL	plasma expander	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	We gave a perfluorochemical oxygen-transport fluid and plasma expander , Fluosol-DA , to seven severely anemic patients before surgery to determine its effectiveness in supplementing oxygen transport .
	manualset3
230188	3	421502	7	NULL	NULL	NULL	NULL	Fluosol-DA 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We gave a perfluorochemical oxygen-transport fluid and plasma expander , Fluosol-DA , to seven severely anemic patients before surgery to determine its effectiveness in supplementing oxygen transport .
	manualset3
230189	4	421502	7	NULL	NULL	0	NULL	seven severely anemic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We gave a perfluorochemical oxygen-transport fluid and plasma expander , Fluosol-DA , to seven severely anemic patients before surgery to determine its effectiveness in supplementing oxygen transport .
	manualset3
230190	5	421502	7	NULL	NULL	0	NULL	surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	We gave a perfluorochemical oxygen-transport fluid and plasma expander , Fluosol-DA , to seven severely anemic patients before surgery to determine its effectiveness in supplementing oxygen transport .
	manualset3
230191	6	421502	7	NULL	NULL	0	NULL	effectiveness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We gave a perfluorochemical oxygen-transport fluid and plasma expander , Fluosol-DA , to seven severely anemic patients before surgery to determine its effectiveness in supplementing oxygen transport .
	manualset3
230192	7	421502	7	NULL	NULL	0	NULL	oxygen transport	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We gave a perfluorochemical oxygen-transport fluid and plasma expander , Fluosol-DA , to seven severely anemic patients before surgery to determine its effectiveness in supplementing oxygen transport .
	manualset3
230193	1	421503	7	NULL	NULL	0	NULL	ideas	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the ideas of E.A. Ernst , it is suggested that anesthesia systems be differentiated according to the underlying principles of construction into rebreathing systems , flow - and valve-controlled non-rebreathing systems , and systems without reservoirs .
	manualset3
230194	2	421503	7	NULL	NULL	0	NULL	E.A. Ernst 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the ideas of E.A. Ernst , it is suggested that anesthesia systems be differentiated according to the underlying principles of construction into rebreathing systems , flow - and valve-controlled non-rebreathing systems , and systems without reservoirs .
	manualset3
230195	3	421503	7	NULL	NULL	NULL	NULL	anesthesia systems	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following the ideas of E.A. Ernst , it is suggested that anesthesia systems be differentiated according to the underlying principles of construction into rebreathing systems , flow - and valve-controlled non-rebreathing systems , and systems without reservoirs .
	manualset3
230196	4	421503	7	NULL	NULL	0	NULL	underlying principles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the ideas of E.A. Ernst , it is suggested that anesthesia systems be differentiated according to the underlying principles of construction into rebreathing systems , flow - and valve-controlled non-rebreathing systems , and systems without reservoirs .
	manualset3
230197	5	421503	7	NULL	NULL	0	NULL	construction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the ideas of E.A. Ernst , it is suggested that anesthesia systems be differentiated according to the underlying principles of construction into rebreathing systems , flow - and valve-controlled non-rebreathing systems , and systems without reservoirs .
	manualset3
230198	6	421503	7	NULL	NULL	0	NULL	rebreathing systems	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the ideas of E.A. Ernst , it is suggested that anesthesia systems be differentiated according to the underlying principles of construction into rebreathing systems , flow - and valve-controlled non-rebreathing systems , and systems without reservoirs .
	manualset3
230199	7	421503	7	NULL	NULL	0	NULL	flow - and valve-controlled non-rebreathing systems	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the ideas of E.A. Ernst , it is suggested that anesthesia systems be differentiated according to the underlying principles of construction into rebreathing systems , flow - and valve-controlled non-rebreathing systems , and systems without reservoirs .
	manualset3
230200	8	421503	7	NULL	NULL	0	NULL	systems without reservoirs 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the ideas of E.A. Ernst , it is suggested that anesthesia systems be differentiated according to the underlying principles of construction into rebreathing systems , flow - and valve-controlled non-rebreathing systems , and systems without reservoirs .
	manualset3
230201	1	421504	7	NULL	NULL	0	NULL	k-space	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Beyond k-space : spectral localization using higher order gradients .
	manualset3
230202	2	421504	7	NULL	NULL	0	NULL	spectral localization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Beyond k-space : spectral localization using higher order gradients .
	manualset3
230203	3	421504	7	NULL	NULL	0	NULL	higher order gradients	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Beyond k-space : spectral localization using higher order gradients .
	manualset3
230204	1	421505	7	NULL	NULL	0	NULL	Symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Symptoms correlated with duration of exposure inside the plant during the honey pack and improved in other environments during that season .
	manualset3
230205	2	421505	7	NULL	NULL	0	NULL	duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Symptoms correlated with duration of exposure inside the plant during the honey pack and improved in other environments during that season .
	manualset3
230206	3	421505	7	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Symptoms correlated with duration of exposure inside the plant during the honey pack and improved in other environments during that season .
	manualset3
230207	4	421505	7	NULL	NULL	0	NULL	 plant 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Symptoms correlated with duration of exposure inside the plant during the honey pack and improved in other environments during that season .
	manualset3
230208	5	421505	7	NULL	NULL	0	NULL	honey pack 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Symptoms correlated with duration of exposure inside the plant during the honey pack and improved in other environments during that season .
	manualset3
230209	6	421505	7	NULL	NULL	0	NULL	environments 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Symptoms correlated with duration of exposure inside the plant during the honey pack and improved in other environments during that season .
	manualset3
230210	7	421505	7	NULL	NULL	0	NULL	 season	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Symptoms correlated with duration of exposure inside the plant during the honey pack and improved in other environments during that season .
	manualset3
230211	1	421506	7	NULL	NULL	0	NULL	factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Included among these factors are : human resources policies ; governmental priorities and planning measures ; professional practices and how they influence the development and structure of the work force ; teaching capacity , and availability of funds and of other resources .
	manualset3
230212	2	421506	7	NULL	NULL	0	NULL	human resources policies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Included among these factors are : human resources policies ; governmental priorities and planning measures ; professional practices and how they influence the development and structure of the work force ; teaching capacity , and availability of funds and of other resources .
	manualset3
230213	3	421506	7	NULL	NULL	0	NULL	governmental priorities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Included among these factors are : human resources policies ; governmental priorities and planning measures ; professional practices and how they influence the development and structure of the work force ; teaching capacity , and availability of funds and of other resources .
	manualset3
230214	4	421506	7	NULL	NULL	0	NULL	planning measures 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Included among these factors are : human resources policies ; governmental priorities and planning measures ; professional practices and how they influence the development and structure of the work force ; teaching capacity , and availability of funds and of other resources .
	manualset3
230215	5	421506	7	NULL	NULL	0	NULL	professional practices	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Included among these factors are : human resources policies ; governmental priorities and planning measures ; professional practices and how they influence the development and structure of the work force ; teaching capacity , and availability of funds and of other resources .
	manualset3
230216	6	421506	7	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Included among these factors are : human resources policies ; governmental priorities and planning measures ; professional practices and how they influence the development and structure of the work force ; teaching capacity , and availability of funds and of other resources .
	manualset3
230217	7	421506	7	NULL	NULL	0	NULL	structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Included among these factors are : human resources policies ; governmental priorities and planning measures ; professional practices and how they influence the development and structure of the work force ; teaching capacity , and availability of funds and of other resources .
	manualset3
230218	8	421506	7	NULL	NULL	0	NULL	work force	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Included among these factors are : human resources policies ; governmental priorities and planning measures ; professional practices and how they influence the development and structure of the work force ; teaching capacity , and availability of funds and of other resources .
	manualset3
230219	9	421506	7	NULL	NULL	0	NULL	teaching capacity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Included among these factors are : human resources policies ; governmental priorities and planning measures ; professional practices and how they influence the development and structure of the work force ; teaching capacity , and availability of funds and of other resources .
	manualset3
230220	10	421506	7	NULL	NULL	0	NULL	availability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Included among these factors are : human resources policies ; governmental priorities and planning measures ; professional practices and how they influence the development and structure of the work force ; teaching capacity , and availability of funds and of other resources .
	manualset3
230221	11	421506	7	NULL	NULL	0	NULL	funds	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Included among these factors are : human resources policies ; governmental priorities and planning measures ; professional practices and how they influence the development and structure of the work force ; teaching capacity , and availability of funds and of other resources .
	manualset3
230222	12	421506	7	NULL	NULL	0	NULL	resources	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Included among these factors are : human resources policies ; governmental priorities and planning measures ; professional practices and how they influence the development and structure of the work force ; teaching capacity , and availability of funds and of other resources .
	manualset3
230223	1	421507	7	NULL	NULL	0	NULL	Sixty HTLV-I seronegative	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty HTLV-I seronegative , age-matched controls showed a normal range of form 63.2 to 480.8 U/mL .
	manualset3
230224	2	421507	7	NULL	NULL	0	NULL	age-matched controls	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty HTLV-I seronegative , age-matched controls showed a normal range of form 63.2 to 480.8 U/mL .
	manualset3
230225	3	421507	7	NULL	NULL	0	NULL	normal range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty HTLV-I seronegative , age-matched controls showed a normal range of form 63.2 to 480.8 U/mL .
	manualset3
230226	4	421507	7	NULL	NULL	0	NULL	form	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty HTLV-I seronegative , age-matched controls showed a normal range of form 63.2 to 480.8 U/mL .
	manualset3
230227	5	421507	7	NULL	NULL	0	NULL	63.2 U/mL	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty HTLV-I seronegative , age-matched controls showed a normal range of form 63.2 to 480.8 U/mL .
	manualset3
230228	6	421507	7	NULL	NULL	0	NULL	480.8 U/mL	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Sixty HTLV-I seronegative , age-matched controls showed a normal range of form 63.2 to 480.8 U/mL .
	manualset3
230229	1	421508	7	NULL	NULL	0	NULL	Courses	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Courses such as this require good administration , as cohesive and supportive tutors ' group , a clear statement of aims , even within a learner-centred framework , and the establishment of clear ground rules to allow the participants to feel safe .
	manualset3
230230	2	421508	7	NULL	NULL	0	NULL	good administration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Courses such as this require good administration , as cohesive and supportive tutors ' group , a clear statement of aims , even within a learner-centred framework , and the establishment of clear ground rules to allow the participants to feel safe .
	manualset3
230231	3	421508	7	NULL	NULL	0	NULL	cohesive tutors ' group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Courses such as this require good administration , as cohesive and supportive tutors ' group , a clear statement of aims , even within a learner-centred framework , and the establishment of clear ground rules to allow the participants to feel safe .
	manualset3
230232	4	421508	7	NULL	NULL	0	NULL	supportive tutors ' group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Courses such as this require good administration , as cohesive and supportive tutors ' group , a clear statement of aims , even within a learner-centred framework , and the establishment of clear ground rules to allow the participants to feel safe .
	manualset3
230233	5	421508	7	NULL	NULL	NULL	NULL	clear statement 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Courses such as this require good administration , as cohesive and supportive tutors ' group , a clear statement of aims , even within a learner-centred framework , and the establishment of clear ground rules to allow the participants to feel safe .
	manualset3
230234	6	421508	7	NULL	NULL	0	NULL	learner-centred framework	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Courses such as this require good administration , as cohesive and supportive tutors ' group , a clear statement of aims , even within a learner-centred framework , and the establishment of clear ground rules to allow the participants to feel safe .
	manualset3
230235	7	421508	7	NULL	NULL	0	NULL	 establishment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Courses such as this require good administration , as cohesive and supportive tutors ' group , a clear statement of aims , even within a learner-centred framework , and the establishment of clear ground rules to allow the participants to feel safe .
	manualset3
230236	8	421508	7	NULL	NULL	0	NULL	clear ground rules	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Courses such as this require good administration , as cohesive and supportive tutors ' group , a clear statement of aims , even within a learner-centred framework , and the establishment of clear ground rules to allow the participants to feel safe .
	manualset3
230237	9	421508	7	NULL	NULL	0	NULL	participants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Courses such as this require good administration , as cohesive and supportive tutors ' group , a clear statement of aims , even within a learner-centred framework , and the establishment of clear ground rules to allow the participants to feel safe .
	manualset3
230238	1	421509	7	NULL	NULL	0	NULL	 setup	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	This setup allows one to obtain better resolution by using a spectral filtering to eliminate noise from the pump pulse , instead of a spatial filtering .
	manualset3
230239	2	421509	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This setup allows one to obtain better resolution by using a spectral filtering to eliminate noise from the pump pulse , instead of a spatial filtering .
	manualset3
230240	3	421509	7	NULL	NULL	0	NULL	better resolution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This setup allows one to obtain better resolution by using a spectral filtering to eliminate noise from the pump pulse , instead of a spatial filtering .
	manualset3
230241	4	421509	7	NULL	NULL	0	NULL	spectral filtering	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This setup allows one to obtain better resolution by using a spectral filtering to eliminate noise from the pump pulse , instead of a spatial filtering .
	manualset3
230242	5	421509	7	NULL	NULL	0	NULL	noise	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	This setup allows one to obtain better resolution by using a spectral filtering to eliminate noise from the pump pulse , instead of a spatial filtering .
	manualset3
230243	6	421509	7	NULL	NULL	0	NULL	pump pulse	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	This setup allows one to obtain better resolution by using a spectral filtering to eliminate noise from the pump pulse , instead of a spatial filtering .
	manualset3
230244	7	421509	7	NULL	NULL	0	NULL	spatial filtering	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This setup allows one to obtain better resolution by using a spectral filtering to eliminate noise from the pump pulse , instead of a spatial filtering .
	manualset3
230245	1	421510	7	NULL	NULL	0	NULL	Annexins I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Annexins I and II were seen in the soluble and particulate fractions of the enamel-related portion but not in the dentin-related portion .
	manualset3
230246	2	421510	7	NULL	NULL	0	NULL	Annexins II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Annexins I and II were seen in the soluble and particulate fractions of the enamel-related portion but not in the dentin-related portion .
	manualset3
230247	3	421510	7	NULL	NULL	NULL	NULL	soluble fractions	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Annexins I and II were seen in the soluble and particulate fractions of the enamel-related portion but not in the dentin-related portion .
	manualset3
230248	4	421510	7	NULL	NULL	NULL	NULL	particulate fractions	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Annexins I and II were seen in the soluble and particulate fractions of the enamel-related portion but not in the dentin-related portion .
	manualset3
230249	5	421510	7	NULL	NULL	0	NULL	 enamel-related portion	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Annexins I and II were seen in the soluble and particulate fractions of the enamel-related portion but not in the dentin-related portion .
	manualset3
230250	6	421510	7	NULL	NULL	0	NULL	dentin-related portion	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Annexins I and II were seen in the soluble and particulate fractions of the enamel-related portion but not in the dentin-related portion .
	manualset3
230251	1	421511	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional patient developed catheter-related C. albicans infection ; the sixth patient developed an infection of cerebrospinal fluid .
	manualset3
230252	2	421511	7	NULL	NULL	0	NULL	catheter-related C. albicans infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional patient developed catheter-related C. albicans infection ; the sixth patient developed an infection of cerebrospinal fluid .
	manualset3
230253	3	421511	7	NULL	NULL	0	NULL	sixth patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional patient developed catheter-related C. albicans infection ; the sixth patient developed an infection of cerebrospinal fluid .
	manualset3
230254	4	421511	7	NULL	NULL	0	NULL	infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional patient developed catheter-related C. albicans infection ; the sixth patient developed an infection of cerebrospinal fluid .
	manualset3
230255	5	421511	7	NULL	NULL	0	NULL	cerebrospinal fluid	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An additional patient developed catheter-related C. albicans infection ; the sixth patient developed an infection of cerebrospinal fluid .
	manualset3
230256	1	421512	7	NULL	NULL	0	NULL	Central venous oxygen saturation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Central venous oxygen saturation and arteriovenous difference of the oxygen content in patients with acute myocardial infarct ) .
	manualset3
230257	2	421512	7	NULL	NULL	0	NULL	arteriovenous difference 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Central venous oxygen saturation and arteriovenous difference of the oxygen content in patients with acute myocardial infarct ) .
	manualset3
230258	3	421512	7	NULL	NULL	0	NULL	 oxygen content 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Central venous oxygen saturation and arteriovenous difference of the oxygen content in patients with acute myocardial infarct ) .
	manualset3
230259	4	421512	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Central venous oxygen saturation and arteriovenous difference of the oxygen content in patients with acute myocardial infarct ) .
	manualset3
230260	5	421512	7	NULL	NULL	0	NULL	acute myocardial infarct 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Central venous oxygen saturation and arteriovenous difference of the oxygen content in patients with acute myocardial infarct ) .
	manualset3
230261	1	421513	7	NULL	NULL	0	NULL	Intra-articular injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-articular injection of interleukin-1 ( IL-1 ) into the knee joints of rabbits produces a synovitis associated with the loss of proteoglycan from the matrix of articular cartilage .
	manualset3
230262	2	421513	7	NULL	NULL	0	NULL	interleukin-1 ( IL-1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-articular injection of interleukin-1 ( IL-1 ) into the knee joints of rabbits produces a synovitis associated with the loss of proteoglycan from the matrix of articular cartilage .
	manualset3
230263	3	421513	7	NULL	NULL	0	NULL	 knee joints	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-articular injection of interleukin-1 ( IL-1 ) into the knee joints of rabbits produces a synovitis associated with the loss of proteoglycan from the matrix of articular cartilage .
	manualset3
230264	4	421513	7	NULL	NULL	0	NULL	rabbits	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-articular injection of interleukin-1 ( IL-1 ) into the knee joints of rabbits produces a synovitis associated with the loss of proteoglycan from the matrix of articular cartilage .
	manualset3
230265	5	421513	7	NULL	NULL	0	NULL	synovitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-articular injection of interleukin-1 ( IL-1 ) into the knee joints of rabbits produces a synovitis associated with the loss of proteoglycan from the matrix of articular cartilage .
	manualset3
230266	6	421513	7	NULL	NULL	0	NULL	loss	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-articular injection of interleukin-1 ( IL-1 ) into the knee joints of rabbits produces a synovitis associated with the loss of proteoglycan from the matrix of articular cartilage .
	manualset3
230267	7	421513	7	NULL	NULL	0	NULL	proteoglycan	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-articular injection of interleukin-1 ( IL-1 ) into the knee joints of rabbits produces a synovitis associated with the loss of proteoglycan from the matrix of articular cartilage .
	manualset3
230268	8	421513	7	NULL	NULL	0	NULL	matrix	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-articular injection of interleukin-1 ( IL-1 ) into the knee joints of rabbits produces a synovitis associated with the loss of proteoglycan from the matrix of articular cartilage .
	manualset3
230269	9	421513	7	NULL	NULL	0	NULL	articular cartilage 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Intra-articular injection of interleukin-1 ( IL-1 ) into the knee joints of rabbits produces a synovitis associated with the loss of proteoglycan from the matrix of articular cartilage .
	manualset3
230270	1	421514	7	NULL	NULL	0	NULL	Collagen-hydroxyapatite ( HA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Collagen-hydroxyapatite ( HA ) scaffolds for the non-viral delivery of a plasmid encoding the osteoinductive protein bone morphogenetic protein ( BMP ) -7 were developed .
	manualset3
230271	2	421514	7	NULL	NULL	NULL	NULL	non-viral delivery	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Collagen-hydroxyapatite ( HA ) scaffolds for the non-viral delivery of a plasmid encoding the osteoinductive protein bone morphogenetic protein ( BMP ) -7 were developed .
	manualset3
230272	3	421514	7	NULL	NULL	0	NULL	plasmid	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Collagen-hydroxyapatite ( HA ) scaffolds for the non-viral delivery of a plasmid encoding the osteoinductive protein bone morphogenetic protein ( BMP ) -7 were developed .
	manualset3
230273	4	421514	7	NULL	NULL	0	NULL	osteoinductive protein bone morphogenetic protein ( BMP ) -7	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Collagen-hydroxyapatite ( HA ) scaffolds for the non-viral delivery of a plasmid encoding the osteoinductive protein bone morphogenetic protein ( BMP ) -7 were developed .
	manualset3
230274	1	421515	7	NULL	NULL	0	NULL	 high degree 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The high degree of amino acid conservation between sFc gammaRIII and other Fc receptors , and similarly between hFc1 and related immunoglobulins , suggest similar structures and modes of association .
	manualset3
230275	2	421515	7	NULL	NULL	0	NULL	amino acid conservation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The high degree of amino acid conservation between sFc gammaRIII and other Fc receptors , and similarly between hFc1 and related immunoglobulins , suggest similar structures and modes of association .
	manualset3
230276	3	421515	7	NULL	NULL	0	NULL	sFc gammaRIII receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The high degree of amino acid conservation between sFc gammaRIII and other Fc receptors , and similarly between hFc1 and related immunoglobulins , suggest similar structures and modes of association .
	manualset3
230277	4	421515	7	NULL	NULL	0	NULL	Fc receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The high degree of amino acid conservation between sFc gammaRIII and other Fc receptors , and similarly between hFc1 and related immunoglobulins , suggest similar structures and modes of association .
	manualset3
230278	5	421515	7	NULL	NULL	0	NULL	hFc1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The high degree of amino acid conservation between sFc gammaRIII and other Fc receptors , and similarly between hFc1 and related immunoglobulins , suggest similar structures and modes of association .
	manualset3
230279	6	421515	7	NULL	NULL	0	NULL	immunoglobulins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The high degree of amino acid conservation between sFc gammaRIII and other Fc receptors , and similarly between hFc1 and related immunoglobulins , suggest similar structures and modes of association .
	manualset3
230280	7	421515	7	NULL	NULL	0	NULL	structures	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The high degree of amino acid conservation between sFc gammaRIII and other Fc receptors , and similarly between hFc1 and related immunoglobulins , suggest similar structures and modes of association .
	manualset3
230281	8	421515	7	NULL	NULL	NULL	NULL	modes of association	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The high degree of amino acid conservation between sFc gammaRIII and other Fc receptors , and similarly between hFc1 and related immunoglobulins , suggest similar structures and modes of association .
	manualset3
230282	1	421516	7	NULL	NULL	0	NULL	qualification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlates of qualification and of study enrollment were determined .
	manualset3
230283	2	421516	7	NULL	NULL	0	NULL	study enrollment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlates of qualification and of study enrollment were determined .
	manualset3
230284	1	421517	7	NULL	NULL	0	NULL	Coronary death 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Coronary death and its forensic evaluation within the scope of the Socialized Accident Insurance of the Federal Republic of Germany ) .
	manualset3
230285	2	421517	7	NULL	NULL	0	NULL	forensic evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Coronary death and its forensic evaluation within the scope of the Socialized Accident Insurance of the Federal Republic of Germany ) .
	manualset3
230286	3	421517	7	NULL	NULL	0	NULL	scope	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Coronary death and its forensic evaluation within the scope of the Socialized Accident Insurance of the Federal Republic of Germany ) .
	manualset3
230287	4	421517	7	NULL	NULL	0	NULL	Socialized Accident Insurance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Coronary death and its forensic evaluation within the scope of the Socialized Accident Insurance of the Federal Republic of Germany ) .
	manualset3
230288	5	421517	7	NULL	NULL	0	NULL	Federal Republic of Germany	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( Coronary death and its forensic evaluation within the scope of the Socialized Accident Insurance of the Federal Republic of Germany ) .
	manualset3
230289	1	421518	7	NULL	NULL	0	NULL	Improved functional ability 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Improved functional ability and independence in activities of daily living for older adults at high risk of hospital readmission : a randomized controlled trial .
	manualset3
230290	2	421518	7	NULL	NULL	0	NULL	activities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Improved functional ability and independence in activities of daily living for older adults at high risk of hospital readmission : a randomized controlled trial .
	manualset3
230291	3	421518	7	NULL	NULL	0	NULL	daily living 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Improved functional ability and independence in activities of daily living for older adults at high risk of hospital readmission : a randomized controlled trial .
	manualset3
230292	4	421518	7	NULL	NULL	0	NULL	older adults 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Improved functional ability and independence in activities of daily living for older adults at high risk of hospital readmission : a randomized controlled trial .
	manualset3
230293	5	421518	7	NULL	NULL	0	NULL	high risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Improved functional ability and independence in activities of daily living for older adults at high risk of hospital readmission : a randomized controlled trial .
	manualset3
230294	6	421518	7	NULL	NULL	0	NULL	hospital readmission	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Improved functional ability and independence in activities of daily living for older adults at high risk of hospital readmission : a randomized controlled trial .
	manualset3
230295	7	421518	7	NULL	NULL	0	NULL	randomized controlled trial	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Improved functional ability and independence in activities of daily living for older adults at high risk of hospital readmission : a randomized controlled trial .
	manualset3
230296	1	421519	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , one should consider tailoring their investigations to suit the radiometal under investigation , and to be mindful where the technology is to be applied ( e.g. imaging organs or disease ) .
	manualset3
230297	2	421519	7	NULL	NULL	0	NULL	investigations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , one should consider tailoring their investigations to suit the radiometal under investigation , and to be mindful where the technology is to be applied ( e.g. imaging organs or disease ) .
	manualset3
230298	3	421519	7	NULL	NULL	0	NULL	radiometal	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	However , one should consider tailoring their investigations to suit the radiometal under investigation , and to be mindful where the technology is to be applied ( e.g. imaging organs or disease ) .
	manualset3
230299	4	421519	7	NULL	NULL	0	NULL	 investigation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , one should consider tailoring their investigations to suit the radiometal under investigation , and to be mindful where the technology is to be applied ( e.g. imaging organs or disease ) .
	manualset3
230300	5	421519	7	NULL	NULL	0	NULL	technology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	However , one should consider tailoring their investigations to suit the radiometal under investigation , and to be mindful where the technology is to be applied ( e.g. imaging organs or disease ) .
	manualset3
230301	6	421519	7	NULL	NULL	0	NULL	 imaging organs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	However , one should consider tailoring their investigations to suit the radiometal under investigation , and to be mindful where the technology is to be applied ( e.g. imaging organs or disease ) .
	manualset3
230302	7	421519	7	NULL	NULL	0	NULL	disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	However , one should consider tailoring their investigations to suit the radiometal under investigation , and to be mindful where the technology is to be applied ( e.g. imaging organs or disease ) .
	manualset3
230303	1	421520	7	NULL	NULL	0	NULL	Evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence suggests that tumor-mediated angiogenesis and enhanced vascular permeability in the peritoneal wall due to high levels of vascular endothelial growth factor play a fundamental role in the pathogenesis of malignant ascites .
	manualset3
230304	2	421520	7	NULL	NULL	0	NULL	tumor-mediated angiogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence suggests that tumor-mediated angiogenesis and enhanced vascular permeability in the peritoneal wall due to high levels of vascular endothelial growth factor play a fundamental role in the pathogenesis of malignant ascites .
	manualset3
230305	3	421520	7	NULL	NULL	0	NULL	vascular permeability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence suggests that tumor-mediated angiogenesis and enhanced vascular permeability in the peritoneal wall due to high levels of vascular endothelial growth factor play a fundamental role in the pathogenesis of malignant ascites .
	manualset3
230306	4	421520	7	NULL	NULL	0	NULL	peritoneal wall	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence suggests that tumor-mediated angiogenesis and enhanced vascular permeability in the peritoneal wall due to high levels of vascular endothelial growth factor play a fundamental role in the pathogenesis of malignant ascites .
	manualset3
230307	5	421520	7	NULL	NULL	0	NULL	high levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence suggests that tumor-mediated angiogenesis and enhanced vascular permeability in the peritoneal wall due to high levels of vascular endothelial growth factor play a fundamental role in the pathogenesis of malignant ascites .
	manualset3
230308	6	421520	7	NULL	NULL	NULL	NULL	vascular endothelial growth factor	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Evidence suggests that tumor-mediated angiogenesis and enhanced vascular permeability in the peritoneal wall due to high levels of vascular endothelial growth factor play a fundamental role in the pathogenesis of malignant ascites .
	manualset3
230309	7	421520	7	NULL	NULL	0	NULL	fundamental role 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence suggests that tumor-mediated angiogenesis and enhanced vascular permeability in the peritoneal wall due to high levels of vascular endothelial growth factor play a fundamental role in the pathogenesis of malignant ascites .
	manualset3
230310	8	421520	7	NULL	NULL	0	NULL	pathogenesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence suggests that tumor-mediated angiogenesis and enhanced vascular permeability in the peritoneal wall due to high levels of vascular endothelial growth factor play a fundamental role in the pathogenesis of malignant ascites .
	manualset3
230311	9	421520	7	NULL	NULL	0	NULL	malignant ascites	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Evidence suggests that tumor-mediated angiogenesis and enhanced vascular permeability in the peritoneal wall due to high levels of vascular endothelial growth factor play a fundamental role in the pathogenesis of malignant ascites .
	manualset3
230312	1	421521	7	NULL	NULL	0	NULL	Statistical analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistical analysis revealed no significant differences among groups for symptoms of anxiety and depression , tendency to worry and worry themes .
	manualset3
230313	2	421521	7	NULL	NULL	0	NULL	no significant differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistical analysis revealed no significant differences among groups for symptoms of anxiety and depression , tendency to worry and worry themes .
	manualset3
230314	3	421521	7	NULL	NULL	0	NULL	 groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistical analysis revealed no significant differences among groups for symptoms of anxiety and depression , tendency to worry and worry themes .
	manualset3
230315	4	421521	7	NULL	NULL	0	NULL	symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistical analysis revealed no significant differences among groups for symptoms of anxiety and depression , tendency to worry and worry themes .
	manualset3
230316	5	421521	7	NULL	NULL	0	NULL	anxiety	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistical analysis revealed no significant differences among groups for symptoms of anxiety and depression , tendency to worry and worry themes .
	manualset3
230317	6	421521	7	NULL	NULL	0	NULL	depression	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistical analysis revealed no significant differences among groups for symptoms of anxiety and depression , tendency to worry and worry themes .
	manualset3
230318	7	421521	7	NULL	NULL	0	NULL	worry themes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Statistical analysis revealed no significant differences among groups for symptoms of anxiety and depression , tendency to worry and worry themes .
	manualset3
230319	1	421522	7	NULL	NULL	0	NULL	acidic FSH 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Least acidic FSH specifically induced the most rapid growth of follicles during preantral development .
	manualset3
230320	2	421522	7	NULL	NULL	0	NULL	rapid growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Least acidic FSH specifically induced the most rapid growth of follicles during preantral development .
	manualset3
230321	3	421522	7	NULL	NULL	0	NULL	follicles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Least acidic FSH specifically induced the most rapid growth of follicles during preantral development .
	manualset3
230322	4	421522	7	NULL	NULL	0	NULL	preantral development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Least acidic FSH specifically induced the most rapid growth of follicles during preantral development .
	manualset3
230323	1	421523	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient was treated surgically and conceived 2 months after the procedure .
	manualset3
230324	2	421523	7	NULL	NULL	0	NULL	2 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient was treated surgically and conceived 2 months after the procedure .
	manualset3
230325	3	421523	7	NULL	NULL	0	NULL	procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patient was treated surgically and conceived 2 months after the procedure .
	manualset3
230326	1	421524	7	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors achieved 57.6 % negativation of the results that gives a reason to propose the use of Azatril ( Balkanpharma ) in the treatment of Chlamydial infection .
	manualset3
230327	2	421524	7	NULL	NULL	0	NULL	 57.6 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors achieved 57.6 % negativation of the results that gives a reason to propose the use of Azatril ( Balkanpharma ) in the treatment of Chlamydial infection .
	manualset3
230328	3	421524	7	NULL	NULL	0	NULL	negativation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors achieved 57.6 % negativation of the results that gives a reason to propose the use of Azatril ( Balkanpharma ) in the treatment of Chlamydial infection .
	manualset3
230329	4	421524	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors achieved 57.6 % negativation of the results that gives a reason to propose the use of Azatril ( Balkanpharma ) in the treatment of Chlamydial infection .
	manualset3
230330	5	421524	7	NULL	NULL	0	NULL	reason	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors achieved 57.6 % negativation of the results that gives a reason to propose the use of Azatril ( Balkanpharma ) in the treatment of Chlamydial infection .
	manualset3
230331	6	421524	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors achieved 57.6 % negativation of the results that gives a reason to propose the use of Azatril ( Balkanpharma ) in the treatment of Chlamydial infection .
	manualset3
230332	7	421524	7	NULL	NULL	0	NULL	Azatril	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors achieved 57.6 % negativation of the results that gives a reason to propose the use of Azatril ( Balkanpharma ) in the treatment of Chlamydial infection .
	manualset3
230333	8	421524	7	NULL	NULL	0	NULL	Balkanpharma	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors achieved 57.6 % negativation of the results that gives a reason to propose the use of Azatril ( Balkanpharma ) in the treatment of Chlamydial infection .
	manualset3
230334	9	421524	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors achieved 57.6 % negativation of the results that gives a reason to propose the use of Azatril ( Balkanpharma ) in the treatment of Chlamydial infection .
	manualset3
230335	10	421524	7	NULL	NULL	0	NULL	Chlamydial infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors achieved 57.6 % negativation of the results that gives a reason to propose the use of Azatril ( Balkanpharma ) in the treatment of Chlamydial infection .
	manualset3
230336	1	421525	7	NULL	NULL	0	NULL	parturition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They increase after parturition , especially in non-lactating mice .
	manualset3
230337	2	421525	7	NULL	NULL	0	NULL	non-lactating mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	They increase after parturition , especially in non-lactating mice .
	manualset3
230338	1	421526	7	NULL	NULL	0	NULL	Data management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Data management and quality assurance for dialysis network .
	manualset3
230339	2	421526	7	NULL	NULL	0	NULL	quality assurance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Data management and quality assurance for dialysis network .
	manualset3
230340	3	421526	7	NULL	NULL	0	NULL	 dialysis network	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Data management and quality assurance for dialysis network .
	manualset3
230341	1	421527	7	NULL	NULL	0	NULL	 note	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A note on the distribution and excretion of antimony in mice treated with sodium p-melaminylphenylstibonate .
	manualset3
230342	2	421527	7	NULL	NULL	NULL	NULL	distribution	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A note on the distribution and excretion of antimony in mice treated with sodium p-melaminylphenylstibonate .
	manualset3
230343	3	421527	7	NULL	NULL	0	NULL	excretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A note on the distribution and excretion of antimony in mice treated with sodium p-melaminylphenylstibonate .
	manualset3
230344	4	421527	7	NULL	NULL	0	NULL	antimony	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A note on the distribution and excretion of antimony in mice treated with sodium p-melaminylphenylstibonate .
	manualset3
230345	5	421527	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A note on the distribution and excretion of antimony in mice treated with sodium p-melaminylphenylstibonate .
	manualset3
230346	6	421527	7	NULL	NULL	0	NULL	sodium p-melaminylphenylstibonate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A note on the distribution and excretion of antimony in mice treated with sodium p-melaminylphenylstibonate .
	manualset3
230347	1	421528	7	NULL	NULL	0	NULL	Development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Development of functional examination of hearing ) .
	manualset3
230348	2	421528	7	NULL	NULL	0	NULL	functional examination 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Development of functional examination of hearing ) .
	manualset3
230349	3	421528	7	NULL	NULL	0	NULL	hearing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Development of functional examination of hearing ) .
	manualset3
230350	1	421529	7	NULL	NULL	0	NULL	adenosine diphosphate sugar pyrophosphatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	An adenosine diphosphate sugar pyrophosphatase ( ASPPase , EC ) has been characterized by using Escherichia coli .
	manualset3
230351	2	421529	7	NULL	NULL	0	NULL	ASPPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	An adenosine diphosphate sugar pyrophosphatase ( ASPPase , EC ) has been characterized by using Escherichia coli .
	manualset3
230352	3	421529	7	NULL	NULL	0	NULL	 EC	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	An adenosine diphosphate sugar pyrophosphatase ( ASPPase , EC ) has been characterized by using Escherichia coli .
	manualset3
230353	4	421529	7	NULL	NULL	0	NULL	Escherichia coli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	An adenosine diphosphate sugar pyrophosphatase ( ASPPase , EC ) has been characterized by using Escherichia coli .
	manualset3
230354	1	421530	7	NULL	NULL	0	NULL	Purification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification of sarcotoxin II , antibacterial proteins of Sarcophaga peregrina ( flesh fly ) larvae .
	manualset3
230355	2	421530	7	NULL	NULL	0	NULL	sarcotoxin II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification of sarcotoxin II , antibacterial proteins of Sarcophaga peregrina ( flesh fly ) larvae .
	manualset3
230356	3	421530	7	NULL	NULL	0	NULL	antibacterial proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Purification of sarcotoxin II , antibacterial proteins of Sarcophaga peregrina ( flesh fly ) larvae .
	manualset3
230357	4	421530	7	NULL	NULL	NULL	NULL	Sarcophaga peregrina ( flesh fly ) larvae	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Purification of sarcotoxin II , antibacterial proteins of Sarcophaga peregrina ( flesh fly ) larvae .
	manualset3
230605	1	421531	7	NULL	NULL	0	NULL	Consistent necropsy findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent necropsy findings in the 4 birds that died were small intestinal crypt cell necrosis and severe bone marrow depletion and necrosis .
	manualset3
230606	2	421531	7	NULL	NULL	0	NULL	4 birds	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent necropsy findings in the 4 birds that died were small intestinal crypt cell necrosis and severe bone marrow depletion and necrosis .
	manualset3
230607	3	421531	7	NULL	NULL	0	NULL	small intestinal crypt cell necrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent necropsy findings in the 4 birds that died were small intestinal crypt cell necrosis and severe bone marrow depletion and necrosis .
	manualset3
230608	4	421531	7	NULL	NULL	0	NULL	severe bone marrow depletion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent necropsy findings in the 4 birds that died were small intestinal crypt cell necrosis and severe bone marrow depletion and necrosis .
	manualset3
230609	5	421531	7	NULL	NULL	0	NULL	necrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent necropsy findings in the 4 birds that died were small intestinal crypt cell necrosis and severe bone marrow depletion and necrosis .
	manualset3
230611	1	421532	7	NULL	NULL	0	NULL	Comparative high-performance liquid chromatographicphotodiode array detection-electrospray ionization-mass spectrometric analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative high-performance liquid chromatographicphotodiode array detection-electrospray ionization-mass spectrometric analyses of plant leaf and insect hemolymph extracts revealed the presence of furostanol saponins in all samples .
	manualset3
230612	2	421532	7	NULL	NULL	0	NULL	 plant leaf 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative high-performance liquid chromatographicphotodiode array detection-electrospray ionization-mass spectrometric analyses of plant leaf and insect hemolymph extracts revealed the presence of furostanol saponins in all samples .
	manualset3
230614	3	421532	7	NULL	NULL	0	NULL	 insect hemolymph extracts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative high-performance liquid chromatographicphotodiode array detection-electrospray ionization-mass spectrometric analyses of plant leaf and insect hemolymph extracts revealed the presence of furostanol saponins in all samples .
	manualset3
230615	4	421532	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative high-performance liquid chromatographicphotodiode array detection-electrospray ionization-mass spectrometric analyses of plant leaf and insect hemolymph extracts revealed the presence of furostanol saponins in all samples .
	manualset3
230616	5	421532	7	NULL	NULL	0	NULL	furostanol saponins	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative high-performance liquid chromatographicphotodiode array detection-electrospray ionization-mass spectrometric analyses of plant leaf and insect hemolymph extracts revealed the presence of furostanol saponins in all samples .
	manualset3
230617	6	421532	7	NULL	NULL	0	NULL	samples	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative high-performance liquid chromatographicphotodiode array detection-electrospray ionization-mass spectrometric analyses of plant leaf and insect hemolymph extracts revealed the presence of furostanol saponins in all samples .
	manualset3
230618	1	421533	7	NULL	NULL	0	NULL	Distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Distribution of cytotoxic and DNA ADP-ribosylating activity in crude extracts from butterflies among the family Pieridae .
	manualset3
230619	2	421533	7	NULL	NULL	0	NULL	cytotoxic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Distribution of cytotoxic and DNA ADP-ribosylating activity in crude extracts from butterflies among the family Pieridae .
	manualset3
230620	3	421533	7	NULL	NULL	NULL	NULL	DNA ADP-ribosylating activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Distribution of cytotoxic and DNA ADP-ribosylating activity in crude extracts from butterflies among the family Pieridae .
	manualset3
230621	4	421533	7	NULL	NULL	0	NULL	 crude extracts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Distribution of cytotoxic and DNA ADP-ribosylating activity in crude extracts from butterflies among the family Pieridae .
	manualset3
230622	5	421533	7	NULL	NULL	0	NULL	butterflies	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Distribution of cytotoxic and DNA ADP-ribosylating activity in crude extracts from butterflies among the family Pieridae .
	manualset3
230623	6	421533	7	NULL	NULL	0	NULL	family Pieridae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Distribution of cytotoxic and DNA ADP-ribosylating activity in crude extracts from butterflies among the family Pieridae .
	manualset3
230624	1	421534	7	NULL	NULL	0	NULL	Centromere-tethered Mps1 pombe homolog ( Mph1 ) kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Centromere-tethered Mps1 pombe homolog ( Mph1 ) kinase is a sufficient marker for recruitment of the spindle checkpoint protein Bub1 , but not Mad1 .
	manualset3
230625	2	421534	7	NULL	NULL	0	NULL	sufficient marker	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Centromere-tethered Mps1 pombe homolog ( Mph1 ) kinase is a sufficient marker for recruitment of the spindle checkpoint protein Bub1 , but not Mad1 .
	manualset3
230626	3	421534	7	NULL	NULL	0	NULL	recruitment	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Centromere-tethered Mps1 pombe homolog ( Mph1 ) kinase is a sufficient marker for recruitment of the spindle checkpoint protein Bub1 , but not Mad1 .
	manualset3
230627	4	421534	7	NULL	NULL	0	NULL	spindle checkpoint protein Bub1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Centromere-tethered Mps1 pombe homolog ( Mph1 ) kinase is a sufficient marker for recruitment of the spindle checkpoint protein Bub1 , but not Mad1 .
	manualset3
230628	5	421534	7	NULL	NULL	0	NULL	Mad1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Centromere-tethered Mps1 pombe homolog ( Mph1 ) kinase is a sufficient marker for recruitment of the spindle checkpoint protein Bub1 , but not Mad1 .
	manualset3
230629	1	421535	7	NULL	NULL	0	NULL	 role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the role of stem cells in carcinogenesis is not well characterised , emerging evidence is providing new insights into this process .
	manualset3
230630	2	421535	7	NULL	NULL	0	NULL	stem cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the role of stem cells in carcinogenesis is not well characterised , emerging evidence is providing new insights into this process .
	manualset3
230631	3	421535	7	NULL	NULL	0	NULL	carcinogenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the role of stem cells in carcinogenesis is not well characterised , emerging evidence is providing new insights into this process .
	manualset3
230632	4	421535	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the role of stem cells in carcinogenesis is not well characterised , emerging evidence is providing new insights into this process .
	manualset3
230633	5	421535	7	NULL	NULL	0	NULL	 new insights	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the role of stem cells in carcinogenesis is not well characterised , emerging evidence is providing new insights into this process .
	manualset3
230634	6	421535	7	NULL	NULL	0	NULL	process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the role of stem cells in carcinogenesis is not well characterised , emerging evidence is providing new insights into this process .
	manualset3
230635	1	421536	7	NULL	NULL	0	NULL	negative brain potential 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It is widely agreed that the negative brain potential elicited at 150-200 ms by a deviant , less intense sound in a repetitive series can be modulated by attention .
	manualset3
230636	2	421536	7	NULL	NULL	0	NULL	150-200 ms	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	It is widely agreed that the negative brain potential elicited at 150-200 ms by a deviant , less intense sound in a repetitive series can be modulated by attention .
	manualset3
230637	3	421536	7	NULL	NULL	0	NULL	deviant	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	It is widely agreed that the negative brain potential elicited at 150-200 ms by a deviant , less intense sound in a repetitive series can be modulated by attention .
	manualset3
230638	4	421536	7	NULL	NULL	0	NULL	less intense sound	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is widely agreed that the negative brain potential elicited at 150-200 ms by a deviant , less intense sound in a repetitive series can be modulated by attention .
	manualset3
230639	5	421536	7	NULL	NULL	0	NULL	repetitive series	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is widely agreed that the negative brain potential elicited at 150-200 ms by a deviant , less intense sound in a repetitive series can be modulated by attention .
	manualset3
230640	6	421536	7	NULL	NULL	0	NULL	attention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is widely agreed that the negative brain potential elicited at 150-200 ms by a deviant , less intense sound in a repetitive series can be modulated by attention .
	manualset3
230641	1	421537	7	NULL	NULL	0	NULL	Ultrasound biomicroscopic assessment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound biomicroscopic assessment of angle parameters in patients with primary angle closure glaucoma undergoing phacoemulsification .
	manualset3
230642	2	421537	7	NULL	NULL	0	NULL	angle parameters	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound biomicroscopic assessment of angle parameters in patients with primary angle closure glaucoma undergoing phacoemulsification .
	manualset3
230643	3	421537	7	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound biomicroscopic assessment of angle parameters in patients with primary angle closure glaucoma undergoing phacoemulsification .
	manualset3
230644	4	421537	7	NULL	NULL	0	NULL	primary angle closure glaucoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound biomicroscopic assessment of angle parameters in patients with primary angle closure glaucoma undergoing phacoemulsification .
	manualset3
230645	5	421537	7	NULL	NULL	0	NULL	phacoemulsification	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound biomicroscopic assessment of angle parameters in patients with primary angle closure glaucoma undergoing phacoemulsification .
	manualset3
230646	1	421538	7	NULL	NULL	0	NULL	adequate intake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An adequate intake of folate during pregnancy , lactation , and infancy is essential for maternal and child health and normal growth .
	manualset3
230647	2	421538	7	NULL	NULL	0	NULL	folate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An adequate intake of folate during pregnancy , lactation , and infancy is essential for maternal and child health and normal growth .
	manualset3
230648	3	421538	7	NULL	NULL	0	NULL	pregnancy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An adequate intake of folate during pregnancy , lactation , and infancy is essential for maternal and child health and normal growth .
	manualset3
230649	4	421538	7	NULL	NULL	NULL	NULL	 lactation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An adequate intake of folate during pregnancy , lactation , and infancy is essential for maternal and child health and normal growth .
	manualset3
230650	5	421538	7	NULL	NULL	0	NULL	 infancy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An adequate intake of folate during pregnancy , lactation , and infancy is essential for maternal and child health and normal growth .
	manualset3
230651	6	421538	7	NULL	NULL	0	NULL	maternal health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An adequate intake of folate during pregnancy , lactation , and infancy is essential for maternal and child health and normal growth .
	manualset3
230652	7	421538	7	NULL	NULL	0	NULL	child health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An adequate intake of folate during pregnancy , lactation , and infancy is essential for maternal and child health and normal growth .
	manualset3
230653	8	421538	7	NULL	NULL	0	NULL	normal growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An adequate intake of folate during pregnancy , lactation , and infancy is essential for maternal and child health and normal growth .
	manualset3
230654	1	421539	7	NULL	NULL	0	NULL	3 - ( 1-methyl-1H-indol-3-yl ) -1 - phenyl-4 - ( 1 - ( 3 - ( piperidin-1-yl ) propyl ) -1 H-pyrazolo ( 3 , 4-b ) pyridine-3-yl ) -1 H-pyrrole-2 , 5 - dione ( YQ36 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	3 - ( 1-methyl-1H-indol-3-yl ) -1 - phenyl-4 - ( 1 - ( 3 - ( piperidin-1-yl ) propyl ) -1 H-pyrazolo ( 3 , 4-b ) pyridine-3-yl ) -1 H-pyrrole-2 , 5 - dione ( YQ36 ) is a novel analog of bisindolylmaleimide , which has been reported to overcome multidrug resistance .
	manualset3
230655	2	421539	7	NULL	NULL	0	NULL	novel analog 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	3 - ( 1-methyl-1H-indol-3-yl ) -1 - phenyl-4 - ( 1 - ( 3 - ( piperidin-1-yl ) propyl ) -1 H-pyrazolo ( 3 , 4-b ) pyridine-3-yl ) -1 H-pyrrole-2 , 5 - dione ( YQ36 ) is a novel analog of bisindolylmaleimide , which has been reported to overcome multidrug resistance .
	manualset3
230656	3	421539	7	NULL	NULL	0	NULL	bisindolylmaleimide 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	3 - ( 1-methyl-1H-indol-3-yl ) -1 - phenyl-4 - ( 1 - ( 3 - ( piperidin-1-yl ) propyl ) -1 H-pyrazolo ( 3 , 4-b ) pyridine-3-yl ) -1 H-pyrrole-2 , 5 - dione ( YQ36 ) is a novel analog of bisindolylmaleimide , which has been reported to overcome multidrug resistance .
	manualset3
230657	4	421539	7	NULL	NULL	0	NULL	multidrug resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	3 - ( 1-methyl-1H-indol-3-yl ) -1 - phenyl-4 - ( 1 - ( 3 - ( piperidin-1-yl ) propyl ) -1 H-pyrazolo ( 3 , 4-b ) pyridine-3-yl ) -1 H-pyrrole-2 , 5 - dione ( YQ36 ) is a novel analog of bisindolylmaleimide , which has been reported to overcome multidrug resistance .
	manualset3
230658	1	421540	7	NULL	NULL	0	NULL	Recordings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recordings of response to free-field stimuli at best frequency were made from single units in the central nucleus of the inferior colliculus of anesthetized cats .
	manualset3
230659	2	421540	7	NULL	NULL	0	NULL	response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recordings of response to free-field stimuli at best frequency were made from single units in the central nucleus of the inferior colliculus of anesthetized cats .
	manualset3
230660	3	421540	7	NULL	NULL	0	NULL	free-field stimuli	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Recordings of response to free-field stimuli at best frequency were made from single units in the central nucleus of the inferior colliculus of anesthetized cats .
	manualset3
230661	4	421540	7	NULL	NULL	0	NULL	best frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recordings of response to free-field stimuli at best frequency were made from single units in the central nucleus of the inferior colliculus of anesthetized cats .
	manualset3
230662	5	421540	7	NULL	NULL	0	NULL	single units 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recordings of response to free-field stimuli at best frequency were made from single units in the central nucleus of the inferior colliculus of anesthetized cats .
	manualset3
230663	6	421540	7	NULL	NULL	0	NULL	central nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Recordings of response to free-field stimuli at best frequency were made from single units in the central nucleus of the inferior colliculus of anesthetized cats .
	manualset3
230664	7	421540	7	NULL	NULL	0	NULL	inferior colliculus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Recordings of response to free-field stimuli at best frequency were made from single units in the central nucleus of the inferior colliculus of anesthetized cats .
	manualset3
230665	8	421540	7	NULL	NULL	0	NULL	anesthetized cats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Recordings of response to free-field stimuli at best frequency were made from single units in the central nucleus of the inferior colliculus of anesthetized cats .
	manualset3
230666	1	421541	7	NULL	NULL	0	NULL	exploration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The exploration consisted of seeking in the synovial membrane ferric pigments by Perls stain , or studying the movements of Fe 59 bound to siderophyllin in the joints .
	manualset3
230667	2	421541	7	NULL	NULL	0	NULL	seeking	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The exploration consisted of seeking in the synovial membrane ferric pigments by Perls stain , or studying the movements of Fe 59 bound to siderophyllin in the joints .
	manualset3
230668	3	421541	7	NULL	NULL	0	NULL	synovial membrane ferric pigments	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The exploration consisted of seeking in the synovial membrane ferric pigments by Perls stain , or studying the movements of Fe 59 bound to siderophyllin in the joints .
	manualset3
230669	4	421541	7	NULL	NULL	0	NULL	Perls stain	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The exploration consisted of seeking in the synovial membrane ferric pigments by Perls stain , or studying the movements of Fe 59 bound to siderophyllin in the joints .
	manualset3
230670	5	421541	7	NULL	NULL	0	NULL	movements 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The exploration consisted of seeking in the synovial membrane ferric pigments by Perls stain , or studying the movements of Fe 59 bound to siderophyllin in the joints .
	manualset3
230671	6	421541	7	NULL	NULL	0	NULL	 Fe 59	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The exploration consisted of seeking in the synovial membrane ferric pigments by Perls stain , or studying the movements of Fe 59 bound to siderophyllin in the joints .
	manualset3
230672	7	421541	7	NULL	NULL	0	NULL	siderophyllin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The exploration consisted of seeking in the synovial membrane ferric pigments by Perls stain , or studying the movements of Fe 59 bound to siderophyllin in the joints .
	manualset3
230673	8	421541	7	NULL	NULL	0	NULL	 joints	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The exploration consisted of seeking in the synovial membrane ferric pigments by Perls stain , or studying the movements of Fe 59 bound to siderophyllin in the joints .
	manualset3
230674	1	421542	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest an inhibitory effect of hyperglycemia on thyroid hormone release .
	manualset3
230675	2	421542	7	NULL	NULL	0	NULL	inhibitory effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest an inhibitory effect of hyperglycemia on thyroid hormone release .
	manualset3
230676	3	421542	7	NULL	NULL	0	NULL	hyperglycemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest an inhibitory effect of hyperglycemia on thyroid hormone release .
	manualset3
230677	4	421542	7	NULL	NULL	0	NULL	thyroid hormone release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggest an inhibitory effect of hyperglycemia on thyroid hormone release .
	manualset3
230763	1	421543	7	NULL	NULL	0	NULL	Expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of protein kinase C isoforms in cultured human retinal pigment epithelial cells .
	manualset3
230764	2	421543	7	NULL	NULL	0	NULL	protein kinase C isoforms	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of protein kinase C isoforms in cultured human retinal pigment epithelial cells .
	manualset3
230765	3	421543	7	NULL	NULL	0	NULL	cultured human retinal pigment epithelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of protein kinase C isoforms in cultured human retinal pigment epithelial cells .
	manualset3
230766	1	421544	7	NULL	NULL	0	NULL	gangliosides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Both gangliosides and SA tended to increase nose poking , number of crossings in the dark-preference test , and time in a lighted compartment .
	manualset3
230767	2	421544	7	NULL	NULL	0	NULL	SA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Both gangliosides and SA tended to increase nose poking , number of crossings in the dark-preference test , and time in a lighted compartment .
	manualset3
230768	3	421544	7	NULL	NULL	0	NULL	nose poking	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Both gangliosides and SA tended to increase nose poking , number of crossings in the dark-preference test , and time in a lighted compartment .
	manualset3
230769	4	421544	7	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Both gangliosides and SA tended to increase nose poking , number of crossings in the dark-preference test , and time in a lighted compartment .
	manualset3
230770	5	421544	7	NULL	NULL	0	NULL	crossings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Both gangliosides and SA tended to increase nose poking , number of crossings in the dark-preference test , and time in a lighted compartment .
	manualset3
230771	6	421544	7	NULL	NULL	0	NULL	dark-preference test 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Both gangliosides and SA tended to increase nose poking , number of crossings in the dark-preference test , and time in a lighted compartment .
	manualset3
230772	7	421544	7	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Both gangliosides and SA tended to increase nose poking , number of crossings in the dark-preference test , and time in a lighted compartment .
	manualset3
230773	8	421544	7	NULL	NULL	0	NULL	lighted compartment 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Both gangliosides and SA tended to increase nose poking , number of crossings in the dark-preference test , and time in a lighted compartment .
	manualset3
230774	1	421545	7	NULL	NULL	0	NULL	Denosumad	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Denosumad , an antibody raised against RANK-Ligand , is a potent bone resorption inhibitor .
	manualset3
230775	2	421545	7	NULL	NULL	0	NULL	antibody	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Denosumad , an antibody raised against RANK-Ligand , is a potent bone resorption inhibitor .
	manualset3
230776	3	421545	7	NULL	NULL	0	NULL	RANK-Ligand	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Denosumad , an antibody raised against RANK-Ligand , is a potent bone resorption inhibitor .
	manualset3
230777	4	421545	7	NULL	NULL	0	NULL	potent bone resorption inhibitor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Denosumad , an antibody raised against RANK-Ligand , is a potent bone resorption inhibitor .
	manualset3
230778	1	421546	7	NULL	NULL	0	NULL	Radio - sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Radio - and thermosensitivity of E. coli K1060 after thiol depletion by diethylmaleate .
	manualset3
230779	2	421546	7	NULL	NULL	0	NULL	thermosensitivity 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Radio - and thermosensitivity of E. coli K1060 after thiol depletion by diethylmaleate .
	manualset3
230780	3	421546	7	NULL	NULL	0	NULL	E. coli K1060	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Radio - and thermosensitivity of E. coli K1060 after thiol depletion by diethylmaleate .
	manualset3
230781	4	421546	7	NULL	NULL	0	NULL	thiol depletion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Radio - and thermosensitivity of E. coli K1060 after thiol depletion by diethylmaleate .
	manualset3
230782	5	421546	7	NULL	NULL	0	NULL	diethylmaleate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Radio - and thermosensitivity of E. coli K1060 after thiol depletion by diethylmaleate .
	manualset3
230783	1	421547	7	NULL	NULL	0	NULL	Examination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Examination of the morphological and proliferative properties of cultures derived from the cerebral cortex and the hypothalamus both in untreated conditions and after treatment with EGF-related ligands illustrates the high plasticity of human astrocytes and their functional heterogeneity according to the cerebral region of origin .
	manualset3
230784	2	421547	7	NULL	NULL	0	NULL	morphological properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Examination of the morphological and proliferative properties of cultures derived from the cerebral cortex and the hypothalamus both in untreated conditions and after treatment with EGF-related ligands illustrates the high plasticity of human astrocytes and their functional heterogeneity according to the cerebral region of origin .
	manualset3
230785	3	421547	7	NULL	NULL	0	NULL	proliferative properties	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Examination of the morphological and proliferative properties of cultures derived from the cerebral cortex and the hypothalamus both in untreated conditions and after treatment with EGF-related ligands illustrates the high plasticity of human astrocytes and their functional heterogeneity according to the cerebral region of origin .
	manualset3
230786	4	421547	7	NULL	NULL	0	NULL	cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Examination of the morphological and proliferative properties of cultures derived from the cerebral cortex and the hypothalamus both in untreated conditions and after treatment with EGF-related ligands illustrates the high plasticity of human astrocytes and their functional heterogeneity according to the cerebral region of origin .
	manualset3
230787	5	421547	7	NULL	NULL	0	NULL	cerebral cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Examination of the morphological and proliferative properties of cultures derived from the cerebral cortex and the hypothalamus both in untreated conditions and after treatment with EGF-related ligands illustrates the high plasticity of human astrocytes and their functional heterogeneity according to the cerebral region of origin .
	manualset3
230788	6	421547	7	NULL	NULL	0	NULL	hypothalamus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Examination of the morphological and proliferative properties of cultures derived from the cerebral cortex and the hypothalamus both in untreated conditions and after treatment with EGF-related ligands illustrates the high plasticity of human astrocytes and their functional heterogeneity according to the cerebral region of origin .
	manualset3
230789	7	421547	7	NULL	NULL	0	NULL	untreated conditions 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Examination of the morphological and proliferative properties of cultures derived from the cerebral cortex and the hypothalamus both in untreated conditions and after treatment with EGF-related ligands illustrates the high plasticity of human astrocytes and their functional heterogeneity according to the cerebral region of origin .
	manualset3
230790	8	421547	7	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Examination of the morphological and proliferative properties of cultures derived from the cerebral cortex and the hypothalamus both in untreated conditions and after treatment with EGF-related ligands illustrates the high plasticity of human astrocytes and their functional heterogeneity according to the cerebral region of origin .
	manualset3
230791	9	421547	7	NULL	NULL	0	NULL	EGF-related ligands	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Examination of the morphological and proliferative properties of cultures derived from the cerebral cortex and the hypothalamus both in untreated conditions and after treatment with EGF-related ligands illustrates the high plasticity of human astrocytes and their functional heterogeneity according to the cerebral region of origin .
	manualset3
230792	10	421547	7	NULL	NULL	0	NULL	high plasticity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Examination of the morphological and proliferative properties of cultures derived from the cerebral cortex and the hypothalamus both in untreated conditions and after treatment with EGF-related ligands illustrates the high plasticity of human astrocytes and their functional heterogeneity according to the cerebral region of origin .
	manualset3
230793	11	421547	7	NULL	NULL	0	NULL	human astrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Examination of the morphological and proliferative properties of cultures derived from the cerebral cortex and the hypothalamus both in untreated conditions and after treatment with EGF-related ligands illustrates the high plasticity of human astrocytes and their functional heterogeneity according to the cerebral region of origin .
	manualset3
230794	12	421547	7	NULL	NULL	0	NULL	 functional heterogeneity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Examination of the morphological and proliferative properties of cultures derived from the cerebral cortex and the hypothalamus both in untreated conditions and after treatment with EGF-related ligands illustrates the high plasticity of human astrocytes and their functional heterogeneity according to the cerebral region of origin .
	manualset3
230795	13	421547	7	NULL	NULL	0	NULL	cerebral region 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Examination of the morphological and proliferative properties of cultures derived from the cerebral cortex and the hypothalamus both in untreated conditions and after treatment with EGF-related ligands illustrates the high plasticity of human astrocytes and their functional heterogeneity according to the cerebral region of origin .
	manualset3
230796	14	421547	7	NULL	NULL	0	NULL	origin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Examination of the morphological and proliferative properties of cultures derived from the cerebral cortex and the hypothalamus both in untreated conditions and after treatment with EGF-related ligands illustrates the high plasticity of human astrocytes and their functional heterogeneity according to the cerebral region of origin .
	manualset3
230797	1	421548	7	NULL	NULL	0	NULL	purpose-designed cannula	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	A purpose-designed cannula for transcervical chorion villus aspiration .
	manualset3
230798	2	421548	7	NULL	NULL	0	NULL	transcervical chorion villus aspiration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A purpose-designed cannula for transcervical chorion villus aspiration .
	manualset3
230799	1	421549	7	NULL	NULL	0	NULL	novel epitope	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel epitope of entactin is present at the mammalian neuromuscular junction .
	manualset3
230800	2	421549	7	NULL	NULL	0	NULL	 entactin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel epitope of entactin is present at the mammalian neuromuscular junction .
	manualset3
230801	3	421549	7	NULL	NULL	0	NULL	 mammalian neuromuscular junction	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel epitope of entactin is present at the mammalian neuromuscular junction .
	manualset3
230802	1	421550	7	NULL	NULL	0	NULL	vital role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We describe the vital role of roboticists and of the group of preverbal infants , who are involved in a robot 's design activity , and we argue that the robot 's social character is intrinsically related to the subtleties of human interactional moves in laboratories of social robotics .
	manualset3
230803	2	421550	7	NULL	NULL	0	NULL	roboticists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We describe the vital role of roboticists and of the group of preverbal infants , who are involved in a robot 's design activity , and we argue that the robot 's social character is intrinsically related to the subtleties of human interactional moves in laboratories of social robotics .
	manualset3
230804	3	421550	7	NULL	NULL	0	NULL	group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We describe the vital role of roboticists and of the group of preverbal infants , who are involved in a robot 's design activity , and we argue that the robot 's social character is intrinsically related to the subtleties of human interactional moves in laboratories of social robotics .
	manualset3
230805	4	421550	7	NULL	NULL	0	NULL	preverbal infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We describe the vital role of roboticists and of the group of preverbal infants , who are involved in a robot 's design activity , and we argue that the robot 's social character is intrinsically related to the subtleties of human interactional moves in laboratories of social robotics .
	manualset3
230806	5	421550	7	NULL	NULL	0	NULL	 robot 's design activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We describe the vital role of roboticists and of the group of preverbal infants , who are involved in a robot 's design activity , and we argue that the robot 's social character is intrinsically related to the subtleties of human interactional moves in laboratories of social robotics .
	manualset3
230807	6	421550	7	NULL	NULL	NULL	NULL	robot 's social character	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We describe the vital role of roboticists and of the group of preverbal infants , who are involved in a robot 's design activity , and we argue that the robot 's social character is intrinsically related to the subtleties of human interactional moves in laboratories of social robotics .
	manualset3
230808	7	421550	7	NULL	NULL	0	NULL	subtleties	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We describe the vital role of roboticists and of the group of preverbal infants , who are involved in a robot 's design activity , and we argue that the robot 's social character is intrinsically related to the subtleties of human interactional moves in laboratories of social robotics .
	manualset3
230809	8	421550	7	NULL	NULL	0	NULL	human interactional moves	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We describe the vital role of roboticists and of the group of preverbal infants , who are involved in a robot 's design activity , and we argue that the robot 's social character is intrinsically related to the subtleties of human interactional moves in laboratories of social robotics .
	manualset3
230810	9	421550	7	NULL	NULL	0	NULL	laboratories	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	We describe the vital role of roboticists and of the group of preverbal infants , who are involved in a robot 's design activity , and we argue that the robot 's social character is intrinsically related to the subtleties of human interactional moves in laboratories of social robotics .
	manualset3
230811	10	421550	7	NULL	NULL	0	NULL	social robotics 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We describe the vital role of roboticists and of the group of preverbal infants , who are involved in a robot 's design activity , and we argue that the robot 's social character is intrinsically related to the subtleties of human interactional moves in laboratories of social robotics .
	manualset3
230813	1	421551	7	NULL	NULL	0	NULL	segments	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These segments reside mainly in the two highly conserved regions of the alpha-subunit in the cytoplasmic domain of Na + , K + - ATPase .
	manualset3
230814	2	421551	7	NULL	NULL	0	NULL	two highly conserved regions	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These segments reside mainly in the two highly conserved regions of the alpha-subunit in the cytoplasmic domain of Na + , K + - ATPase .
	manualset3
230815	3	421551	7	NULL	NULL	0	NULL	alpha-subunit	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These segments reside mainly in the two highly conserved regions of the alpha-subunit in the cytoplasmic domain of Na + , K + - ATPase .
	manualset3
230816	4	421551	7	NULL	NULL	0	NULL	cytoplasmic domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These segments reside mainly in the two highly conserved regions of the alpha-subunit in the cytoplasmic domain of Na + , K + - ATPase .
	manualset3
230817	5	421551	7	NULL	NULL	0	NULL	Na + , K + - ATPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These segments reside mainly in the two highly conserved regions of the alpha-subunit in the cytoplasmic domain of Na + , K + - ATPase .
	manualset3
230818	1	421552	7	NULL	NULL	0	NULL	Increased abundance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased abundance of PAH biodegradation genes was detected by functional gene array in the monitoring well located at the rear end of the biostimulated area , which indicated that air sparging and nutrient infiltration enhanced the intrinsic , aerobic PAH biodegradation .
	manualset3
230819	2	421552	7	NULL	NULL	0	NULL	PAH biodegradation genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased abundance of PAH biodegradation genes was detected by functional gene array in the monitoring well located at the rear end of the biostimulated area , which indicated that air sparging and nutrient infiltration enhanced the intrinsic , aerobic PAH biodegradation .
	manualset3
230820	3	421552	7	NULL	NULL	0	NULL	functional gene array	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased abundance of PAH biodegradation genes was detected by functional gene array in the monitoring well located at the rear end of the biostimulated area , which indicated that air sparging and nutrient infiltration enhanced the intrinsic , aerobic PAH biodegradation .
	manualset3
230823	4	421552	7	NULL	NULL	0	NULL	rear end	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased abundance of PAH biodegradation genes was detected by functional gene array in the monitoring well located at the rear end of the biostimulated area , which indicated that air sparging and nutrient infiltration enhanced the intrinsic , aerobic PAH biodegradation .
	manualset3
230824	5	421552	7	NULL	NULL	0	NULL	biostimulated area	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased abundance of PAH biodegradation genes was detected by functional gene array in the monitoring well located at the rear end of the biostimulated area , which indicated that air sparging and nutrient infiltration enhanced the intrinsic , aerobic PAH biodegradation .
	manualset3
230825	6	421552	7	NULL	NULL	0	NULL	air sparging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased abundance of PAH biodegradation genes was detected by functional gene array in the monitoring well located at the rear end of the biostimulated area , which indicated that air sparging and nutrient infiltration enhanced the intrinsic , aerobic PAH biodegradation .
	manualset3
230826	7	421552	7	NULL	NULL	0	NULL	nutrient infiltration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased abundance of PAH biodegradation genes was detected by functional gene array in the monitoring well located at the rear end of the biostimulated area , which indicated that air sparging and nutrient infiltration enhanced the intrinsic , aerobic PAH biodegradation .
	manualset3
230827	8	421552	7	NULL	NULL	0	NULL	intrinsic , aerobic PAH biodegradation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Increased abundance of PAH biodegradation genes was detected by functional gene array in the monitoring well located at the rear end of the biostimulated area , which indicated that air sparging and nutrient infiltration enhanced the intrinsic , aerobic PAH biodegradation .
	manualset3
230829	1	421553	7	NULL	NULL	0	NULL	VIP	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Is VIP a key neuropeptide in achalasia ?
	manualset3
230830	2	421553	7	NULL	NULL	0	NULL	neuropeptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Is VIP a key neuropeptide in achalasia ?
	manualset3
230831	3	421553	7	NULL	NULL	0	NULL	achalasia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Is VIP a key neuropeptide in achalasia ?
	manualset3
230832	1	421554	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that ionic coupling is neither an inevitable nor an immediate consequence of adhesion .
	manualset3
230834	2	421554	7	NULL	NULL	0	NULL	ionic coupling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that ionic coupling is neither an inevitable nor an immediate consequence of adhesion .
	manualset3
230835	3	421554	7	NULL	NULL	0	NULL	adhesion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that ionic coupling is neither an inevitable nor an immediate consequence of adhesion .
	manualset3
230837	1	421555	7	NULL	NULL	0	NULL	Variants	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Variants of the beta 1 , 3-galactosyltransferase CgtB from the bacterium Campylobacter jejuni have distinct acceptor specificities .
	manualset3
230839	2	421555	7	NULL	NULL	0	NULL	beta 1 , 3-galactosyltransferase CgtB	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Variants of the beta 1 , 3-galactosyltransferase CgtB from the bacterium Campylobacter jejuni have distinct acceptor specificities .
	manualset3
230841	3	421555	7	NULL	NULL	0	NULL	bacterium Campylobacter jejuni	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Variants of the beta 1 , 3-galactosyltransferase CgtB from the bacterium Campylobacter jejuni have distinct acceptor specificities .
	manualset3
230842	4	421555	7	NULL	NULL	0	NULL	acceptor specificities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Variants of the beta 1 , 3-galactosyltransferase CgtB from the bacterium Campylobacter jejuni have distinct acceptor specificities .
	manualset3
230845	1	421556	7	NULL	NULL	0	NULL	effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect on somatostatin and VIP is partly mediated via cholinergic neurons .
	manualset3
230846	2	421556	7	NULL	NULL	0	NULL	somatostatin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect on somatostatin and VIP is partly mediated via cholinergic neurons .
	manualset3
230847	3	421556	7	NULL	NULL	0	NULL	VIP	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect on somatostatin and VIP is partly mediated via cholinergic neurons .
	manualset3
230848	4	421556	7	NULL	NULL	0	NULL	cholinergic neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect on somatostatin and VIP is partly mediated via cholinergic neurons .
	manualset3
230850	1	421557	7	NULL	NULL	0	NULL	 ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of creatine phosphate ( PCr ) to inorganic phosphate ( Pi ) ( PCr/Pi ) showed a precipitous decrease in parallel with changes in electroencephalographic ( EEG ) amplitude in severe strokes during ischemia as well as during recirculation .
	manualset3
230851	2	421557	7	NULL	NULL	0	NULL	creatine phosphate ( PCr )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of creatine phosphate ( PCr ) to inorganic phosphate ( Pi ) ( PCr/Pi ) showed a precipitous decrease in parallel with changes in electroencephalographic ( EEG ) amplitude in severe strokes during ischemia as well as during recirculation .
	manualset3
230852	3	421557	7	NULL	NULL	0	NULL	 inorganic phosphate ( Pi )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of creatine phosphate ( PCr ) to inorganic phosphate ( Pi ) ( PCr/Pi ) showed a precipitous decrease in parallel with changes in electroencephalographic ( EEG ) amplitude in severe strokes during ischemia as well as during recirculation .
	manualset3
230854	4	421557	7	NULL	NULL	0	NULL	PCr/Pi	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of creatine phosphate ( PCr ) to inorganic phosphate ( Pi ) ( PCr/Pi ) showed a precipitous decrease in parallel with changes in electroencephalographic ( EEG ) amplitude in severe strokes during ischemia as well as during recirculation .
	manualset3
230855	5	421557	7	NULL	NULL	0	NULL	electroencephalographic ( EEG ) amplitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of creatine phosphate ( PCr ) to inorganic phosphate ( Pi ) ( PCr/Pi ) showed a precipitous decrease in parallel with changes in electroencephalographic ( EEG ) amplitude in severe strokes during ischemia as well as during recirculation .
	manualset3
230856	6	421557	7	NULL	NULL	0	NULL	severe strokes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of creatine phosphate ( PCr ) to inorganic phosphate ( Pi ) ( PCr/Pi ) showed a precipitous decrease in parallel with changes in electroencephalographic ( EEG ) amplitude in severe strokes during ischemia as well as during recirculation .
	manualset3
230858	7	421557	7	NULL	NULL	0	NULL	 ischemia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of creatine phosphate ( PCr ) to inorganic phosphate ( Pi ) ( PCr/Pi ) showed a precipitous decrease in parallel with changes in electroencephalographic ( EEG ) amplitude in severe strokes during ischemia as well as during recirculation .
	manualset3
230859	8	421557	7	NULL	NULL	0	NULL	recirculation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of creatine phosphate ( PCr ) to inorganic phosphate ( Pi ) ( PCr/Pi ) showed a precipitous decrease in parallel with changes in electroencephalographic ( EEG ) amplitude in severe strokes during ischemia as well as during recirculation .
	manualset3
230860	9	421557	7	NULL	NULL	0	NULL	precipitous decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of creatine phosphate ( PCr ) to inorganic phosphate ( Pi ) ( PCr/Pi ) showed a precipitous decrease in parallel with changes in electroencephalographic ( EEG ) amplitude in severe strokes during ischemia as well as during recirculation .
	manualset3
230861	10	421557	7	NULL	NULL	0	NULL	changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The ratio of creatine phosphate ( PCr ) to inorganic phosphate ( Pi ) ( PCr/Pi ) showed a precipitous decrease in parallel with changes in electroencephalographic ( EEG ) amplitude in severe strokes during ischemia as well as during recirculation .
	manualset3
230866	1	421558	7	NULL	NULL	0	NULL	Cav-1 deficient mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	As such , Cav-1 deficient mice show a dramatically reduced mitochondrial reserve capacity .
	manualset3
230867	2	421558	7	NULL	NULL	0	NULL	mitochondrial reserve capacity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As such , Cav-1 deficient mice show a dramatically reduced mitochondrial reserve capacity .
	manualset3
230868	1	421559	7	NULL	NULL	0	NULL	Specific ways	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific ways a resident can enhance his or her `` academic marketability '' include 1 ) involvement in research , 2 ) establishment of a track record of productivity via scholarly writing , 3 ) awareness of the literature in the specialty , 4 ) involvement in specialty organizations and hospital committees , 5 ) competition for national awards , 6 ) gaining education skills , 7 ) developing an academic niche , and 8 ) fellowship training .
	manualset3
230869	2	421559	7	NULL	NULL	0	NULL	resident	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific ways a resident can enhance his or her `` academic marketability '' include 1 ) involvement in research , 2 ) establishment of a track record of productivity via scholarly writing , 3 ) awareness of the literature in the specialty , 4 ) involvement in specialty organizations and hospital committees , 5 ) competition for national awards , 6 ) gaining education skills , 7 ) developing an academic niche , and 8 ) fellowship training .
	manualset3
230870	3	421559	7	NULL	NULL	0	NULL	academic marketability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific ways a resident can enhance his or her `` academic marketability '' include 1 ) involvement in research , 2 ) establishment of a track record of productivity via scholarly writing , 3 ) awareness of the literature in the specialty , 4 ) involvement in specialty organizations and hospital committees , 5 ) competition for national awards , 6 ) gaining education skills , 7 ) developing an academic niche , and 8 ) fellowship training .
	manualset3
230871	4	421559	7	NULL	NULL	0	NULL	involvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific ways a resident can enhance his or her `` academic marketability '' include 1 ) involvement in research , 2 ) establishment of a track record of productivity via scholarly writing , 3 ) awareness of the literature in the specialty , 4 ) involvement in specialty organizations and hospital committees , 5 ) competition for national awards , 6 ) gaining education skills , 7 ) developing an academic niche , and 8 ) fellowship training .
	manualset3
230872	5	421559	7	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific ways a resident can enhance his or her `` academic marketability '' include 1 ) involvement in research , 2 ) establishment of a track record of productivity via scholarly writing , 3 ) awareness of the literature in the specialty , 4 ) involvement in specialty organizations and hospital committees , 5 ) competition for national awards , 6 ) gaining education skills , 7 ) developing an academic niche , and 8 ) fellowship training .
	manualset3
230874	6	421559	7	NULL	NULL	0	NULL	establishment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific ways a resident can enhance his or her `` academic marketability '' include 1 ) involvement in research , 2 ) establishment of a track record of productivity via scholarly writing , 3 ) awareness of the literature in the specialty , 4 ) involvement in specialty organizations and hospital committees , 5 ) competition for national awards , 6 ) gaining education skills , 7 ) developing an academic niche , and 8 ) fellowship training .
	manualset3
230875	7	421559	7	NULL	NULL	0	NULL	track record 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific ways a resident can enhance his or her `` academic marketability '' include 1 ) involvement in research , 2 ) establishment of a track record of productivity via scholarly writing , 3 ) awareness of the literature in the specialty , 4 ) involvement in specialty organizations and hospital committees , 5 ) competition for national awards , 6 ) gaining education skills , 7 ) developing an academic niche , and 8 ) fellowship training .
	manualset3
230876	8	421559	7	NULL	NULL	0	NULL	productivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific ways a resident can enhance his or her `` academic marketability '' include 1 ) involvement in research , 2 ) establishment of a track record of productivity via scholarly writing , 3 ) awareness of the literature in the specialty , 4 ) involvement in specialty organizations and hospital committees , 5 ) competition for national awards , 6 ) gaining education skills , 7 ) developing an academic niche , and 8 ) fellowship training .
	manualset3
230877	9	421559	7	NULL	NULL	0	NULL	scholarly writing 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific ways a resident can enhance his or her `` academic marketability '' include 1 ) involvement in research , 2 ) establishment of a track record of productivity via scholarly writing , 3 ) awareness of the literature in the specialty , 4 ) involvement in specialty organizations and hospital committees , 5 ) competition for national awards , 6 ) gaining education skills , 7 ) developing an academic niche , and 8 ) fellowship training .
	manualset3
230878	10	421559	7	NULL	NULL	0	NULL	awareness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific ways a resident can enhance his or her `` academic marketability '' include 1 ) involvement in research , 2 ) establishment of a track record of productivity via scholarly writing , 3 ) awareness of the literature in the specialty , 4 ) involvement in specialty organizations and hospital committees , 5 ) competition for national awards , 6 ) gaining education skills , 7 ) developing an academic niche , and 8 ) fellowship training .
	manualset3
230879	11	421559	7	NULL	NULL	0	NULL	 literature 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific ways a resident can enhance his or her `` academic marketability '' include 1 ) involvement in research , 2 ) establishment of a track record of productivity via scholarly writing , 3 ) awareness of the literature in the specialty , 4 ) involvement in specialty organizations and hospital committees , 5 ) competition for national awards , 6 ) gaining education skills , 7 ) developing an academic niche , and 8 ) fellowship training .
	manualset3
230880	12	421559	7	NULL	NULL	0	NULL	specialty	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific ways a resident can enhance his or her `` academic marketability '' include 1 ) involvement in research , 2 ) establishment of a track record of productivity via scholarly writing , 3 ) awareness of the literature in the specialty , 4 ) involvement in specialty organizations and hospital committees , 5 ) competition for national awards , 6 ) gaining education skills , 7 ) developing an academic niche , and 8 ) fellowship training .
	manualset3
230881	13	421559	7	NULL	NULL	0	NULL	involvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific ways a resident can enhance his or her `` academic marketability '' include 1 ) involvement in research , 2 ) establishment of a track record of productivity via scholarly writing , 3 ) awareness of the literature in the specialty , 4 ) involvement in specialty organizations and hospital committees , 5 ) competition for national awards , 6 ) gaining education skills , 7 ) developing an academic niche , and 8 ) fellowship training .
	manualset3
230882	14	421559	7	NULL	NULL	0	NULL	specialty organizations	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific ways a resident can enhance his or her `` academic marketability '' include 1 ) involvement in research , 2 ) establishment of a track record of productivity via scholarly writing , 3 ) awareness of the literature in the specialty , 4 ) involvement in specialty organizations and hospital committees , 5 ) competition for national awards , 6 ) gaining education skills , 7 ) developing an academic niche , and 8 ) fellowship training .
	manualset3
230883	15	421559	7	NULL	NULL	0	NULL	hospital committees	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific ways a resident can enhance his or her `` academic marketability '' include 1 ) involvement in research , 2 ) establishment of a track record of productivity via scholarly writing , 3 ) awareness of the literature in the specialty , 4 ) involvement in specialty organizations and hospital committees , 5 ) competition for national awards , 6 ) gaining education skills , 7 ) developing an academic niche , and 8 ) fellowship training .
	manualset3
230884	16	421559	7	NULL	NULL	0	NULL	competition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific ways a resident can enhance his or her `` academic marketability '' include 1 ) involvement in research , 2 ) establishment of a track record of productivity via scholarly writing , 3 ) awareness of the literature in the specialty , 4 ) involvement in specialty organizations and hospital committees , 5 ) competition for national awards , 6 ) gaining education skills , 7 ) developing an academic niche , and 8 ) fellowship training .
	manualset3
230885	17	421559	7	NULL	NULL	0	NULL	 national awards	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific ways a resident can enhance his or her `` academic marketability '' include 1 ) involvement in research , 2 ) establishment of a track record of productivity via scholarly writing , 3 ) awareness of the literature in the specialty , 4 ) involvement in specialty organizations and hospital committees , 5 ) competition for national awards , 6 ) gaining education skills , 7 ) developing an academic niche , and 8 ) fellowship training .
	manualset3
230886	18	421559	7	NULL	NULL	0	NULL	gaining education skills	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific ways a resident can enhance his or her `` academic marketability '' include 1 ) involvement in research , 2 ) establishment of a track record of productivity via scholarly writing , 3 ) awareness of the literature in the specialty , 4 ) involvement in specialty organizations and hospital committees , 5 ) competition for national awards , 6 ) gaining education skills , 7 ) developing an academic niche , and 8 ) fellowship training .
	manualset3
230887	19	421559	7	NULL	NULL	0	NULL	developing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific ways a resident can enhance his or her `` academic marketability '' include 1 ) involvement in research , 2 ) establishment of a track record of productivity via scholarly writing , 3 ) awareness of the literature in the specialty , 4 ) involvement in specialty organizations and hospital committees , 5 ) competition for national awards , 6 ) gaining education skills , 7 ) developing an academic niche , and 8 ) fellowship training .
	manualset3
230888	20	421559	7	NULL	NULL	0	NULL	academic niche	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific ways a resident can enhance his or her `` academic marketability '' include 1 ) involvement in research , 2 ) establishment of a track record of productivity via scholarly writing , 3 ) awareness of the literature in the specialty , 4 ) involvement in specialty organizations and hospital committees , 5 ) competition for national awards , 6 ) gaining education skills , 7 ) developing an academic niche , and 8 ) fellowship training .
	manualset3
230889	21	421559	7	NULL	NULL	0	NULL	fellowship training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specific ways a resident can enhance his or her `` academic marketability '' include 1 ) involvement in research , 2 ) establishment of a track record of productivity via scholarly writing , 3 ) awareness of the literature in the specialty , 4 ) involvement in specialty organizations and hospital committees , 5 ) competition for national awards , 6 ) gaining education skills , 7 ) developing an academic niche , and 8 ) fellowship training .
	manualset3
230890	1	421560	7	NULL	NULL	0	NULL	partial correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	No , or only partial correlation with the results obtained with voltammetry was found with MK 212 , cinanserin , metergoline and quipazine .
	manualset3
230891	2	421560	7	NULL	NULL	0	NULL	 results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	No , or only partial correlation with the results obtained with voltammetry was found with MK 212 , cinanserin , metergoline and quipazine .
	manualset3
230892	3	421560	7	NULL	NULL	0	NULL	voltammetry	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	No , or only partial correlation with the results obtained with voltammetry was found with MK 212 , cinanserin , metergoline and quipazine .
	manualset3
230894	4	421560	7	NULL	NULL	0	NULL	MK 212	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	No , or only partial correlation with the results obtained with voltammetry was found with MK 212 , cinanserin , metergoline and quipazine .
	manualset3
230895	5	421560	7	NULL	NULL	0	NULL	cinanserin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	No , or only partial correlation with the results obtained with voltammetry was found with MK 212 , cinanserin , metergoline and quipazine .
	manualset3
230896	6	421560	7	NULL	NULL	0	NULL	metergoline 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	No , or only partial correlation with the results obtained with voltammetry was found with MK 212 , cinanserin , metergoline and quipazine .
	manualset3
230898	7	421560	7	NULL	NULL	0	NULL	quipazine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	No , or only partial correlation with the results obtained with voltammetry was found with MK 212 , cinanserin , metergoline and quipazine .
	manualset3
230911	1	421561	7	NULL	NULL	0	NULL	HA alkaloid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	HA and HO , cephalotaxus alkaloids are a new class of active compounds of plant origin which may differ from the vinca alkaloids in the mechanism of antitumor activity .
	manualset3
230912	2	421561	7	NULL	NULL	0	NULL	HO alkaloid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	HA and HO , cephalotaxus alkaloids are a new class of active compounds of plant origin which may differ from the vinca alkaloids in the mechanism of antitumor activity .
	manualset3
230913	3	421561	7	NULL	NULL	0	NULL	cephalotaxus alkaloids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	HA and HO , cephalotaxus alkaloids are a new class of active compounds of plant origin which may differ from the vinca alkaloids in the mechanism of antitumor activity .
	manualset3
230914	4	421561	7	NULL	NULL	0	NULL	new class	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	HA and HO , cephalotaxus alkaloids are a new class of active compounds of plant origin which may differ from the vinca alkaloids in the mechanism of antitumor activity .
	manualset3
230915	5	421561	7	NULL	NULL	0	NULL	active compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	HA and HO , cephalotaxus alkaloids are a new class of active compounds of plant origin which may differ from the vinca alkaloids in the mechanism of antitumor activity .
	manualset3
230916	6	421561	7	NULL	NULL	0	NULL	plant origin 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	HA and HO , cephalotaxus alkaloids are a new class of active compounds of plant origin which may differ from the vinca alkaloids in the mechanism of antitumor activity .
	manualset3
230917	7	421561	7	NULL	NULL	0	NULL	vinca alkaloids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	HA and HO , cephalotaxus alkaloids are a new class of active compounds of plant origin which may differ from the vinca alkaloids in the mechanism of antitumor activity .
	manualset3
230930	8	421561	7	NULL	NULL	0	NULL	mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HA and HO , cephalotaxus alkaloids are a new class of active compounds of plant origin which may differ from the vinca alkaloids in the mechanism of antitumor activity .
	manualset3
230931	9	421561	7	NULL	NULL	0	NULL	antitumor activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HA and HO , cephalotaxus alkaloids are a new class of active compounds of plant origin which may differ from the vinca alkaloids in the mechanism of antitumor activity .
	manualset3
230932	1	421562	7	NULL	NULL	0	NULL	Catalytic properties	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Catalytic properties of chloroplast F1-ATPase modified at catalytic or noncatalytic sites by 2-azido adenine nucleotides .
	manualset3
230933	2	421562	7	NULL	NULL	0	NULL	chloroplast F1-ATPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Catalytic properties of chloroplast F1-ATPase modified at catalytic or noncatalytic sites by 2-azido adenine nucleotides .
	manualset3
230934	3	421562	7	NULL	NULL	0	NULL	catalytic sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Catalytic properties of chloroplast F1-ATPase modified at catalytic or noncatalytic sites by 2-azido adenine nucleotides .
	manualset3
230935	4	421562	7	NULL	NULL	0	NULL	noncatalytic sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Catalytic properties of chloroplast F1-ATPase modified at catalytic or noncatalytic sites by 2-azido adenine nucleotides .
	manualset3
230936	5	421562	7	NULL	NULL	0	NULL	 2-azido adenine nucleotides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Catalytic properties of chloroplast F1-ATPase modified at catalytic or noncatalytic sites by 2-azido adenine nucleotides .
	manualset3
230937	1	421563	7	NULL	NULL	NULL	NULL	Regular inhalation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Regular inhalation of both DSCG and beta 2 stimulant is recommended for the treatment of severe asthma in the guideline which was made in 1993 .
	manualset3
230938	2	421563	7	NULL	NULL	0	NULL	DSCG 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular inhalation of both DSCG and beta 2 stimulant is recommended for the treatment of severe asthma in the guideline which was made in 1993 .
	manualset3
230939	3	421563	7	NULL	NULL	0	NULL	beta 2 stimulant	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular inhalation of both DSCG and beta 2 stimulant is recommended for the treatment of severe asthma in the guideline which was made in 1993 .
	manualset3
230940	4	421563	7	NULL	NULL	0	NULL	 treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular inhalation of both DSCG and beta 2 stimulant is recommended for the treatment of severe asthma in the guideline which was made in 1993 .
	manualset3
230941	5	421563	7	NULL	NULL	0	NULL	severe asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular inhalation of both DSCG and beta 2 stimulant is recommended for the treatment of severe asthma in the guideline which was made in 1993 .
	manualset3
230942	6	421563	7	NULL	NULL	0	NULL	guideline	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular inhalation of both DSCG and beta 2 stimulant is recommended for the treatment of severe asthma in the guideline which was made in 1993 .
	manualset3
230943	7	421563	7	NULL	NULL	0	NULL	1993 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Regular inhalation of both DSCG and beta 2 stimulant is recommended for the treatment of severe asthma in the guideline which was made in 1993 .
	manualset3
230944	1	421564	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews current knowledge of FVIIa interaction with TF and EPCR on cell surfaces with a specific focus on how these interactions may contribute to FVIIa and TF clearance , thereby regulating TF-FVIIa activity .
	manualset3
230945	2	421564	7	NULL	NULL	0	NULL	current knowledge 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews current knowledge of FVIIa interaction with TF and EPCR on cell surfaces with a specific focus on how these interactions may contribute to FVIIa and TF clearance , thereby regulating TF-FVIIa activity .
	manualset3
230946	3	421564	7	NULL	NULL	0	NULL	FVIIa interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews current knowledge of FVIIa interaction with TF and EPCR on cell surfaces with a specific focus on how these interactions may contribute to FVIIa and TF clearance , thereby regulating TF-FVIIa activity .
	manualset3
230947	4	421564	7	NULL	NULL	0	NULL	TF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews current knowledge of FVIIa interaction with TF and EPCR on cell surfaces with a specific focus on how these interactions may contribute to FVIIa and TF clearance , thereby regulating TF-FVIIa activity .
	manualset3
230948	5	421564	7	NULL	NULL	0	NULL	EPCR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews current knowledge of FVIIa interaction with TF and EPCR on cell surfaces with a specific focus on how these interactions may contribute to FVIIa and TF clearance , thereby regulating TF-FVIIa activity .
	manualset3
230949	6	421564	7	NULL	NULL	0	NULL	cell surfaces	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews current knowledge of FVIIa interaction with TF and EPCR on cell surfaces with a specific focus on how these interactions may contribute to FVIIa and TF clearance , thereby regulating TF-FVIIa activity .
	manualset3
230950	7	421564	7	NULL	NULL	0	NULL	specific focus	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews current knowledge of FVIIa interaction with TF and EPCR on cell surfaces with a specific focus on how these interactions may contribute to FVIIa and TF clearance , thereby regulating TF-FVIIa activity .
	manualset3
230951	8	421564	7	NULL	NULL	0	NULL	interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews current knowledge of FVIIa interaction with TF and EPCR on cell surfaces with a specific focus on how these interactions may contribute to FVIIa and TF clearance , thereby regulating TF-FVIIa activity .
	manualset3
230952	9	421564	7	NULL	NULL	0	NULL	FVIIa clearance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews current knowledge of FVIIa interaction with TF and EPCR on cell surfaces with a specific focus on how these interactions may contribute to FVIIa and TF clearance , thereby regulating TF-FVIIa activity .
	manualset3
230953	10	421564	7	NULL	NULL	0	NULL	TF clearance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews current knowledge of FVIIa interaction with TF and EPCR on cell surfaces with a specific focus on how these interactions may contribute to FVIIa and TF clearance , thereby regulating TF-FVIIa activity .
	manualset3
230954	11	421564	7	NULL	NULL	0	NULL	TF-FVIIa activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This article reviews current knowledge of FVIIa interaction with TF and EPCR on cell surfaces with a specific focus on how these interactions may contribute to FVIIa and TF clearance , thereby regulating TF-FVIIa activity .
	manualset3
230955	1	421565	7	NULL	NULL	0	NULL	Policy makers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Policy makers and planners in Bangladesh must be made aware that such sex biases exist and that these patterns are exacerbated during food shortages .
	manualset3
230956	2	421565	7	NULL	NULL	0	NULL	planners	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Policy makers and planners in Bangladesh must be made aware that such sex biases exist and that these patterns are exacerbated during food shortages .
	manualset3
230957	3	421565	7	NULL	NULL	0	NULL	Bangladesh	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Policy makers and planners in Bangladesh must be made aware that such sex biases exist and that these patterns are exacerbated during food shortages .
	manualset3
230958	4	421565	7	NULL	NULL	0	NULL	sex biases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Policy makers and planners in Bangladesh must be made aware that such sex biases exist and that these patterns are exacerbated during food shortages .
	manualset3
230959	5	421565	7	NULL	NULL	0	NULL	 patterns 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Policy makers and planners in Bangladesh must be made aware that such sex biases exist and that these patterns are exacerbated during food shortages .
	manualset3
230960	6	421565	7	NULL	NULL	0	NULL	food shortages	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Policy makers and planners in Bangladesh must be made aware that such sex biases exist and that these patterns are exacerbated during food shortages .
	manualset3
230961	1	421566	7	NULL	NULL	0	NULL	availability 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	To estimate the availability of systemically administered vancomycin to the interstitial fluid in the lung , we have used a sheep model with a chronic pulmonary lymph fistula to collect simultaneously series of plasma and pulmonary lymph specimens during a 6-h period after an intravenous dose of vancomycin ( 7 mg/kg ) .
	manualset3
230962	2	421566	7	NULL	NULL	0	NULL	vancomycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	To estimate the availability of systemically administered vancomycin to the interstitial fluid in the lung , we have used a sheep model with a chronic pulmonary lymph fistula to collect simultaneously series of plasma and pulmonary lymph specimens during a 6-h period after an intravenous dose of vancomycin ( 7 mg/kg ) .
	manualset3
230963	3	421566	7	NULL	NULL	0	NULL	interstitial fluid	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To estimate the availability of systemically administered vancomycin to the interstitial fluid in the lung , we have used a sheep model with a chronic pulmonary lymph fistula to collect simultaneously series of plasma and pulmonary lymph specimens during a 6-h period after an intravenous dose of vancomycin ( 7 mg/kg ) .
	manualset3
230964	4	421566	7	NULL	NULL	0	NULL	 lung	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To estimate the availability of systemically administered vancomycin to the interstitial fluid in the lung , we have used a sheep model with a chronic pulmonary lymph fistula to collect simultaneously series of plasma and pulmonary lymph specimens during a 6-h period after an intravenous dose of vancomycin ( 7 mg/kg ) .
	manualset3
230965	5	421566	7	NULL	NULL	0	NULL	sheep model	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To estimate the availability of systemically administered vancomycin to the interstitial fluid in the lung , we have used a sheep model with a chronic pulmonary lymph fistula to collect simultaneously series of plasma and pulmonary lymph specimens during a 6-h period after an intravenous dose of vancomycin ( 7 mg/kg ) .
	manualset3
230966	6	421566	7	NULL	NULL	0	NULL	chronic pulmonary lymph fistula	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To estimate the availability of systemically administered vancomycin to the interstitial fluid in the lung , we have used a sheep model with a chronic pulmonary lymph fistula to collect simultaneously series of plasma and pulmonary lymph specimens during a 6-h period after an intravenous dose of vancomycin ( 7 mg/kg ) .
	manualset3
230967	7	421566	7	NULL	NULL	0	NULL	plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To estimate the availability of systemically administered vancomycin to the interstitial fluid in the lung , we have used a sheep model with a chronic pulmonary lymph fistula to collect simultaneously series of plasma and pulmonary lymph specimens during a 6-h period after an intravenous dose of vancomycin ( 7 mg/kg ) .
	manualset3
230968	8	421566	7	NULL	NULL	0	NULL	pulmonary lymph specimens	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	To estimate the availability of systemically administered vancomycin to the interstitial fluid in the lung , we have used a sheep model with a chronic pulmonary lymph fistula to collect simultaneously series of plasma and pulmonary lymph specimens during a 6-h period after an intravenous dose of vancomycin ( 7 mg/kg ) .
	manualset3
230969	9	421566	7	NULL	NULL	0	NULL	6-h period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	To estimate the availability of systemically administered vancomycin to the interstitial fluid in the lung , we have used a sheep model with a chronic pulmonary lymph fistula to collect simultaneously series of plasma and pulmonary lymph specimens during a 6-h period after an intravenous dose of vancomycin ( 7 mg/kg ) .
	manualset3
230970	10	421566	7	NULL	NULL	0	NULL	intravenous dose 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	To estimate the availability of systemically administered vancomycin to the interstitial fluid in the lung , we have used a sheep model with a chronic pulmonary lymph fistula to collect simultaneously series of plasma and pulmonary lymph specimens during a 6-h period after an intravenous dose of vancomycin ( 7 mg/kg ) .
	manualset3
230971	11	421566	7	NULL	NULL	0	NULL	vancomycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	To estimate the availability of systemically administered vancomycin to the interstitial fluid in the lung , we have used a sheep model with a chronic pulmonary lymph fistula to collect simultaneously series of plasma and pulmonary lymph specimens during a 6-h period after an intravenous dose of vancomycin ( 7 mg/kg ) .
	manualset3
230972	12	421566	7	NULL	NULL	0	NULL	7 mg/kg 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	To estimate the availability of systemically administered vancomycin to the interstitial fluid in the lung , we have used a sheep model with a chronic pulmonary lymph fistula to collect simultaneously series of plasma and pulmonary lymph specimens during a 6-h period after an intravenous dose of vancomycin ( 7 mg/kg ) .
	manualset3
230973	1	421567	7	NULL	NULL	0	NULL	G-banding 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using G-banding and SKY , the GM7 cell line was identified as near-triploid with a large number of structural and numerical abnormalities .
	manualset3
230974	2	421567	7	NULL	NULL	0	NULL	SKY	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using G-banding and SKY , the GM7 cell line was identified as near-triploid with a large number of structural and numerical abnormalities .
	manualset3
230975	3	421567	7	NULL	NULL	0	NULL	GM7 cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using G-banding and SKY , the GM7 cell line was identified as near-triploid with a large number of structural and numerical abnormalities .
	manualset3
230976	4	421567	7	NULL	NULL	0	NULL	near-triploid	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using G-banding and SKY , the GM7 cell line was identified as near-triploid with a large number of structural and numerical abnormalities .
	manualset3
230977	5	421567	7	NULL	NULL	0	NULL	 large number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using G-banding and SKY , the GM7 cell line was identified as near-triploid with a large number of structural and numerical abnormalities .
	manualset3
230978	6	421567	7	NULL	NULL	0	NULL	structural abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using G-banding and SKY , the GM7 cell line was identified as near-triploid with a large number of structural and numerical abnormalities .
	manualset3
230979	7	421567	7	NULL	NULL	0	NULL	numerical abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Using G-banding and SKY , the GM7 cell line was identified as near-triploid with a large number of structural and numerical abnormalities .
	manualset3
230980	1	421568	7	NULL	NULL	0	NULL	algorithm	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	An algorithm may be used in the analysis of elevated transaminase levels : after elimination of the most frequent causes of hepatitis ( alcoholic hepatitis , chronic hepatitis B and C ) and some rare conditions ( autoimmune hepatitis , alpha 1-antitrypsin deficiency , hemochromatosis and Wilson 's disease ) , the diagnosis will often be nonalcoholic steatohepatitis .
	manualset3
230981	2	421568	7	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An algorithm may be used in the analysis of elevated transaminase levels : after elimination of the most frequent causes of hepatitis ( alcoholic hepatitis , chronic hepatitis B and C ) and some rare conditions ( autoimmune hepatitis , alpha 1-antitrypsin deficiency , hemochromatosis and Wilson 's disease ) , the diagnosis will often be nonalcoholic steatohepatitis .
	manualset3
230982	3	421568	7	NULL	NULL	0	NULL	elevated transaminase levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An algorithm may be used in the analysis of elevated transaminase levels : after elimination of the most frequent causes of hepatitis ( alcoholic hepatitis , chronic hepatitis B and C ) and some rare conditions ( autoimmune hepatitis , alpha 1-antitrypsin deficiency , hemochromatosis and Wilson 's disease ) , the diagnosis will often be nonalcoholic steatohepatitis .
	manualset3
230983	4	421568	7	NULL	NULL	0	NULL	elimination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An algorithm may be used in the analysis of elevated transaminase levels : after elimination of the most frequent causes of hepatitis ( alcoholic hepatitis , chronic hepatitis B and C ) and some rare conditions ( autoimmune hepatitis , alpha 1-antitrypsin deficiency , hemochromatosis and Wilson 's disease ) , the diagnosis will often be nonalcoholic steatohepatitis .
	manualset3
230984	5	421568	7	NULL	NULL	0	NULL	frequent causes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An algorithm may be used in the analysis of elevated transaminase levels : after elimination of the most frequent causes of hepatitis ( alcoholic hepatitis , chronic hepatitis B and C ) and some rare conditions ( autoimmune hepatitis , alpha 1-antitrypsin deficiency , hemochromatosis and Wilson 's disease ) , the diagnosis will often be nonalcoholic steatohepatitis .
	manualset3
230985	6	421568	7	NULL	NULL	0	NULL	hepatitis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	An algorithm may be used in the analysis of elevated transaminase levels : after elimination of the most frequent causes of hepatitis ( alcoholic hepatitis , chronic hepatitis B and C ) and some rare conditions ( autoimmune hepatitis , alpha 1-antitrypsin deficiency , hemochromatosis and Wilson 's disease ) , the diagnosis will often be nonalcoholic steatohepatitis .
	manualset3
230986	7	421568	7	NULL	NULL	0	NULL	alcoholic hepatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	An algorithm may be used in the analysis of elevated transaminase levels : after elimination of the most frequent causes of hepatitis ( alcoholic hepatitis , chronic hepatitis B and C ) and some rare conditions ( autoimmune hepatitis , alpha 1-antitrypsin deficiency , hemochromatosis and Wilson 's disease ) , the diagnosis will often be nonalcoholic steatohepatitis .
	manualset3
230987	8	421568	7	NULL	NULL	0	NULL	chronic hepatitis B 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	An algorithm may be used in the analysis of elevated transaminase levels : after elimination of the most frequent causes of hepatitis ( alcoholic hepatitis , chronic hepatitis B and C ) and some rare conditions ( autoimmune hepatitis , alpha 1-antitrypsin deficiency , hemochromatosis and Wilson 's disease ) , the diagnosis will often be nonalcoholic steatohepatitis .
	manualset3
230988	9	421568	7	NULL	NULL	0	NULL	chronic hepatitis C	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	An algorithm may be used in the analysis of elevated transaminase levels : after elimination of the most frequent causes of hepatitis ( alcoholic hepatitis , chronic hepatitis B and C ) and some rare conditions ( autoimmune hepatitis , alpha 1-antitrypsin deficiency , hemochromatosis and Wilson 's disease ) , the diagnosis will often be nonalcoholic steatohepatitis .
	manualset3
230989	10	421568	7	NULL	NULL	0	NULL	rare conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An algorithm may be used in the analysis of elevated transaminase levels : after elimination of the most frequent causes of hepatitis ( alcoholic hepatitis , chronic hepatitis B and C ) and some rare conditions ( autoimmune hepatitis , alpha 1-antitrypsin deficiency , hemochromatosis and Wilson 's disease ) , the diagnosis will often be nonalcoholic steatohepatitis .
	manualset3
230990	11	421568	7	NULL	NULL	0	NULL	autoimmune hepatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	An algorithm may be used in the analysis of elevated transaminase levels : after elimination of the most frequent causes of hepatitis ( alcoholic hepatitis , chronic hepatitis B and C ) and some rare conditions ( autoimmune hepatitis , alpha 1-antitrypsin deficiency , hemochromatosis and Wilson 's disease ) , the diagnosis will often be nonalcoholic steatohepatitis .
	manualset3
230991	12	421568	7	NULL	NULL	0	NULL	alpha 1-antitrypsin deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An algorithm may be used in the analysis of elevated transaminase levels : after elimination of the most frequent causes of hepatitis ( alcoholic hepatitis , chronic hepatitis B and C ) and some rare conditions ( autoimmune hepatitis , alpha 1-antitrypsin deficiency , hemochromatosis and Wilson 's disease ) , the diagnosis will often be nonalcoholic steatohepatitis .
	manualset3
230992	13	421568	7	NULL	NULL	0	NULL	hemochromatosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	An algorithm may be used in the analysis of elevated transaminase levels : after elimination of the most frequent causes of hepatitis ( alcoholic hepatitis , chronic hepatitis B and C ) and some rare conditions ( autoimmune hepatitis , alpha 1-antitrypsin deficiency , hemochromatosis and Wilson 's disease ) , the diagnosis will often be nonalcoholic steatohepatitis .
	manualset3
230993	14	421568	7	NULL	NULL	0	NULL	Wilson 's disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	An algorithm may be used in the analysis of elevated transaminase levels : after elimination of the most frequent causes of hepatitis ( alcoholic hepatitis , chronic hepatitis B and C ) and some rare conditions ( autoimmune hepatitis , alpha 1-antitrypsin deficiency , hemochromatosis and Wilson 's disease ) , the diagnosis will often be nonalcoholic steatohepatitis .
	manualset3
230994	15	421568	7	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An algorithm may be used in the analysis of elevated transaminase levels : after elimination of the most frequent causes of hepatitis ( alcoholic hepatitis , chronic hepatitis B and C ) and some rare conditions ( autoimmune hepatitis , alpha 1-antitrypsin deficiency , hemochromatosis and Wilson 's disease ) , the diagnosis will often be nonalcoholic steatohepatitis .
	manualset3
230995	16	421568	7	NULL	NULL	0	NULL	nonalcoholic steatohepatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	An algorithm may be used in the analysis of elevated transaminase levels : after elimination of the most frequent causes of hepatitis ( alcoholic hepatitis , chronic hepatitis B and C ) and some rare conditions ( autoimmune hepatitis , alpha 1-antitrypsin deficiency , hemochromatosis and Wilson 's disease ) , the diagnosis will often be nonalcoholic steatohepatitis .
	manualset3
230996	1	421569	7	NULL	NULL	0	NULL	coordination complex 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The coordination complex between 1 and zinc chloride 4 is described according to its single-crystal X-ray structure .
	manualset3
230997	2	421569	7	NULL	NULL	0	NULL	1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The coordination complex between 1 and zinc chloride 4 is described according to its single-crystal X-ray structure .
	manualset3
230998	3	421569	7	NULL	NULL	0	NULL	zinc chloride 4 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The coordination complex between 1 and zinc chloride 4 is described according to its single-crystal X-ray structure .
	manualset3
230999	4	421569	7	NULL	NULL	0	NULL	single-crystal X-ray structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The coordination complex between 1 and zinc chloride 4 is described according to its single-crystal X-ray structure .
	manualset3
231000	1	421570	7	NULL	NULL	0	NULL	Senile alteration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Senile alteration of hemodynamics in surgery of abdominal aneurysm ) .
	manualset3
231001	2	421570	7	NULL	NULL	0	NULL	hemodynamics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Senile alteration of hemodynamics in surgery of abdominal aneurysm ) .
	manualset3
231002	3	421570	7	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Senile alteration of hemodynamics in surgery of abdominal aneurysm ) .
	manualset3
231003	4	421570	7	NULL	NULL	0	NULL	abdominal aneurysm	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Senile alteration of hemodynamics in surgery of abdominal aneurysm ) .
	manualset3
231004	1	421571	7	NULL	NULL	0	NULL	Fluorescent imaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescent imaging using fluorescent styryl-dye FM4-64 revealed that chronic blockade of KCNQ2/3 channels decreased endocytosis but facilitated exocytosis .
	manualset3
231005	2	421571	7	NULL	NULL	0	NULL	fluorescent styryl-dye FM4-64	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescent imaging using fluorescent styryl-dye FM4-64 revealed that chronic blockade of KCNQ2/3 channels decreased endocytosis but facilitated exocytosis .
	manualset3
231006	3	421571	7	NULL	NULL	0	NULL	chronic blockade	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescent imaging using fluorescent styryl-dye FM4-64 revealed that chronic blockade of KCNQ2/3 channels decreased endocytosis but facilitated exocytosis .
	manualset3
231007	4	421571	7	NULL	NULL	0	NULL	KCNQ2/3 channels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescent imaging using fluorescent styryl-dye FM4-64 revealed that chronic blockade of KCNQ2/3 channels decreased endocytosis but facilitated exocytosis .
	manualset3
231008	5	421571	7	NULL	NULL	0	NULL	endocytosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescent imaging using fluorescent styryl-dye FM4-64 revealed that chronic blockade of KCNQ2/3 channels decreased endocytosis but facilitated exocytosis .
	manualset3
231009	6	421571	7	NULL	NULL	0	NULL	exocytosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescent imaging using fluorescent styryl-dye FM4-64 revealed that chronic blockade of KCNQ2/3 channels decreased endocytosis but facilitated exocytosis .
	manualset3
231010	1	421572	7	NULL	NULL	0	NULL	structural patterns	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural patterns were classified into monomers , dimers , and trimers , which were supposed to be generated from a precursor guaiazulene and followed by side-chain and nucleus oxidation and oxidative rearrangement .
	manualset3
231011	2	421572	7	NULL	NULL	0	NULL	monomers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural patterns were classified into monomers , dimers , and trimers , which were supposed to be generated from a precursor guaiazulene and followed by side-chain and nucleus oxidation and oxidative rearrangement .
	manualset3
231012	3	421572	7	NULL	NULL	0	NULL	dimers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural patterns were classified into monomers , dimers , and trimers , which were supposed to be generated from a precursor guaiazulene and followed by side-chain and nucleus oxidation and oxidative rearrangement .
	manualset3
231013	4	421572	7	NULL	NULL	0	NULL	trimers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural patterns were classified into monomers , dimers , and trimers , which were supposed to be generated from a precursor guaiazulene and followed by side-chain and nucleus oxidation and oxidative rearrangement .
	manualset3
231014	5	421572	7	NULL	NULL	0	NULL	precursor guaiazulene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural patterns were classified into monomers , dimers , and trimers , which were supposed to be generated from a precursor guaiazulene and followed by side-chain and nucleus oxidation and oxidative rearrangement .
	manualset3
231015	6	421572	7	NULL	NULL	0	NULL	side-chain 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural patterns were classified into monomers , dimers , and trimers , which were supposed to be generated from a precursor guaiazulene and followed by side-chain and nucleus oxidation and oxidative rearrangement .
	manualset3
231016	7	421572	7	NULL	NULL	0	NULL	nucleus oxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural patterns were classified into monomers , dimers , and trimers , which were supposed to be generated from a precursor guaiazulene and followed by side-chain and nucleus oxidation and oxidative rearrangement .
	manualset3
231017	8	421572	7	NULL	NULL	0	NULL	oxidative rearrangement	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural patterns were classified into monomers , dimers , and trimers , which were supposed to be generated from a precursor guaiazulene and followed by side-chain and nucleus oxidation and oxidative rearrangement .
	manualset3
231018	1	421573	7	NULL	NULL	0	NULL	experimental study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An experimental study with silver impregnation methods .
	manualset3
231019	2	421573	7	NULL	NULL	0	NULL	silver impregnation methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An experimental study with silver impregnation methods .
	manualset3
231020	1	421574	7	NULL	NULL	0	NULL	 effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of recombinant human Tumor Necrosis Factor ( rHu-TNF , PT-050 ) , an antitumor agent , on the cardiovascular , gastrointestinal , renal and blood functions were examined in experimental animals .
	manualset3
231021	2	421574	7	NULL	NULL	0	NULL	recombinant human Tumor Necrosis Factor ( rHu-TNF , PT-050 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of recombinant human Tumor Necrosis Factor ( rHu-TNF , PT-050 ) , an antitumor agent , on the cardiovascular , gastrointestinal , renal and blood functions were examined in experimental animals .
	manualset3
231022	3	421574	7	NULL	NULL	0	NULL	antitumor agent	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of recombinant human Tumor Necrosis Factor ( rHu-TNF , PT-050 ) , an antitumor agent , on the cardiovascular , gastrointestinal , renal and blood functions were examined in experimental animals .
	manualset3
231023	4	421574	7	NULL	NULL	0	NULL	cardiovascular functions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of recombinant human Tumor Necrosis Factor ( rHu-TNF , PT-050 ) , an antitumor agent , on the cardiovascular , gastrointestinal , renal and blood functions were examined in experimental animals .
	manualset3
231024	5	421574	7	NULL	NULL	0	NULL	gastrointestinal functions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of recombinant human Tumor Necrosis Factor ( rHu-TNF , PT-050 ) , an antitumor agent , on the cardiovascular , gastrointestinal , renal and blood functions were examined in experimental animals .
	manualset3
231025	6	421574	7	NULL	NULL	0	NULL	renal functions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of recombinant human Tumor Necrosis Factor ( rHu-TNF , PT-050 ) , an antitumor agent , on the cardiovascular , gastrointestinal , renal and blood functions were examined in experimental animals .
	manualset3
231026	7	421574	7	NULL	NULL	0	NULL	blood functions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of recombinant human Tumor Necrosis Factor ( rHu-TNF , PT-050 ) , an antitumor agent , on the cardiovascular , gastrointestinal , renal and blood functions were examined in experimental animals .
	manualset3
231027	8	421574	7	NULL	NULL	0	NULL	experimental animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of recombinant human Tumor Necrosis Factor ( rHu-TNF , PT-050 ) , an antitumor agent , on the cardiovascular , gastrointestinal , renal and blood functions were examined in experimental animals .
	manualset3
231028	1	421575	7	NULL	NULL	0	NULL	selector-like gene functions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to these selector-like gene functions , Sp1 and btd are also required during larval stages for the growth of the leg .
	manualset3
231029	2	421575	7	NULL	NULL	0	NULL	Sp1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to these selector-like gene functions , Sp1 and btd are also required during larval stages for the growth of the leg .
	manualset3
231030	3	421575	7	NULL	NULL	0	NULL	btd	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to these selector-like gene functions , Sp1 and btd are also required during larval stages for the growth of the leg .
	manualset3
231031	4	421575	7	NULL	NULL	0	NULL	larval stages	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to these selector-like gene functions , Sp1 and btd are also required during larval stages for the growth of the leg .
	manualset3
231032	5	421575	7	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to these selector-like gene functions , Sp1 and btd are also required during larval stages for the growth of the leg .
	manualset3
231033	6	421575	7	NULL	NULL	0	NULL	leg	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition to these selector-like gene functions , Sp1 and btd are also required during larval stages for the growth of the leg .
	manualset3
231034	1	421576	7	NULL	NULL	0	NULL	murine endotoxin shock model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In the murine endotoxin shock model , pirfenidone potently inhibited the production of the proinflammatory cytokines , TNF-alpha , interferon-gamma , and interleukin-6 , but enhanced the production of the anti-inflammatory cytokine , interleukin-10 .
	manualset3
231035	2	421576	7	NULL	NULL	0	NULL	pirfenidone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the murine endotoxin shock model , pirfenidone potently inhibited the production of the proinflammatory cytokines , TNF-alpha , interferon-gamma , and interleukin-6 , but enhanced the production of the anti-inflammatory cytokine , interleukin-10 .
	manualset3
231036	3	421576	7	NULL	NULL	0	NULL	production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the murine endotoxin shock model , pirfenidone potently inhibited the production of the proinflammatory cytokines , TNF-alpha , interferon-gamma , and interleukin-6 , but enhanced the production of the anti-inflammatory cytokine , interleukin-10 .
	manualset3
231037	4	421576	7	NULL	NULL	0	NULL	 proinflammatory cytokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the murine endotoxin shock model , pirfenidone potently inhibited the production of the proinflammatory cytokines , TNF-alpha , interferon-gamma , and interleukin-6 , but enhanced the production of the anti-inflammatory cytokine , interleukin-10 .
	manualset3
231038	5	421576	7	NULL	NULL	0	NULL	TNF-alpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the murine endotoxin shock model , pirfenidone potently inhibited the production of the proinflammatory cytokines , TNF-alpha , interferon-gamma , and interleukin-6 , but enhanced the production of the anti-inflammatory cytokine , interleukin-10 .
	manualset3
231039	6	421576	7	NULL	NULL	0	NULL	 interferon-gamma	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the murine endotoxin shock model , pirfenidone potently inhibited the production of the proinflammatory cytokines , TNF-alpha , interferon-gamma , and interleukin-6 , but enhanced the production of the anti-inflammatory cytokine , interleukin-10 .
	manualset3
231040	7	421576	7	NULL	NULL	0	NULL	interleukin-6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the murine endotoxin shock model , pirfenidone potently inhibited the production of the proinflammatory cytokines , TNF-alpha , interferon-gamma , and interleukin-6 , but enhanced the production of the anti-inflammatory cytokine , interleukin-10 .
	manualset3
231041	8	421576	7	NULL	NULL	0	NULL	production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the murine endotoxin shock model , pirfenidone potently inhibited the production of the proinflammatory cytokines , TNF-alpha , interferon-gamma , and interleukin-6 , but enhanced the production of the anti-inflammatory cytokine , interleukin-10 .
	manualset3
231042	9	421576	7	NULL	NULL	0	NULL	anti-inflammatory cytokine	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the murine endotoxin shock model , pirfenidone potently inhibited the production of the proinflammatory cytokines , TNF-alpha , interferon-gamma , and interleukin-6 , but enhanced the production of the anti-inflammatory cytokine , interleukin-10 .
	manualset3
231043	10	421576	7	NULL	NULL	0	NULL	interleukin-10	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In the murine endotoxin shock model , pirfenidone potently inhibited the production of the proinflammatory cytokines , TNF-alpha , interferon-gamma , and interleukin-6 , but enhanced the production of the anti-inflammatory cytokine , interleukin-10 .
	manualset3
231044	1	421577	7	NULL	NULL	0	NULL	Pre-operative imaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-operative imaging of rectal cancer and its impact on surgical performance and treatment outcome .
	manualset3
231045	2	421577	7	NULL	NULL	0	NULL	rectal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-operative imaging of rectal cancer and its impact on surgical performance and treatment outcome .
	manualset3
231046	3	421577	7	NULL	NULL	0	NULL	surgical performance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-operative imaging of rectal cancer and its impact on surgical performance and treatment outcome .
	manualset3
231047	4	421577	7	NULL	NULL	0	NULL	treatment outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-operative imaging of rectal cancer and its impact on surgical performance and treatment outcome .
	manualset3
233188	5	421577	7	NULL	NULL	0	NULL	impact	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre-operative imaging of rectal cancer and its impact on surgical performance and treatment outcome .
	manualset3
231048	1	421578	7	NULL	NULL	0	NULL	alkali-thermotolerant extracellular protease	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	An alkali-thermotolerant extracellular protease from a newly isolated Streptomyces sp .
	manualset3
231049	2	421578	7	NULL	NULL	0	NULL	newly isolated Streptomyces sp	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	An alkali-thermotolerant extracellular protease from a newly isolated Streptomyces sp .
	manualset3
231050	1	421579	7	NULL	NULL	0	NULL	unfolding process 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The unfolding process has been found to be reversible in the case of fluoro alcohol/water mixtures , while no such reversibility was found in the case of sodium dodecyl sulfate .
	manualset3
231051	2	421579	7	NULL	NULL	0	NULL	case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The unfolding process has been found to be reversible in the case of fluoro alcohol/water mixtures , while no such reversibility was found in the case of sodium dodecyl sulfate .
	manualset3
231052	3	421579	7	NULL	NULL	0	NULL	fluoro alcohol/water mixtures	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The unfolding process has been found to be reversible in the case of fluoro alcohol/water mixtures , while no such reversibility was found in the case of sodium dodecyl sulfate .
	manualset3
231053	4	421579	7	NULL	NULL	0	NULL	reversibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The unfolding process has been found to be reversible in the case of fluoro alcohol/water mixtures , while no such reversibility was found in the case of sodium dodecyl sulfate .
	manualset3
231054	5	421579	7	NULL	NULL	0	NULL	case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The unfolding process has been found to be reversible in the case of fluoro alcohol/water mixtures , while no such reversibility was found in the case of sodium dodecyl sulfate .
	manualset3
231055	6	421579	7	NULL	NULL	0	NULL	sodium dodecyl sulfate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The unfolding process has been found to be reversible in the case of fluoro alcohol/water mixtures , while no such reversibility was found in the case of sodium dodecyl sulfate .
	manualset3
231056	1	421580	7	NULL	NULL	0	NULL	low-frequency alpha band	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A low-frequency alpha band appeared immediately after eye closing , but it later disappeared and was replaced by a new development of a high-frequency alpha band 4-5 min after the onset of VAB .
	manualset3
231057	2	421580	7	NULL	NULL	0	NULL	eye closing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A low-frequency alpha band appeared immediately after eye closing , but it later disappeared and was replaced by a new development of a high-frequency alpha band 4-5 min after the onset of VAB .
	manualset3
231058	3	421580	7	NULL	NULL	0	NULL	new development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A low-frequency alpha band appeared immediately after eye closing , but it later disappeared and was replaced by a new development of a high-frequency alpha band 4-5 min after the onset of VAB .
	manualset3
231059	4	421580	7	NULL	NULL	0	NULL	high-frequency alpha band 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A low-frequency alpha band appeared immediately after eye closing , but it later disappeared and was replaced by a new development of a high-frequency alpha band 4-5 min after the onset of VAB .
	manualset3
231060	5	421580	7	NULL	NULL	0	NULL	4-5 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A low-frequency alpha band appeared immediately after eye closing , but it later disappeared and was replaced by a new development of a high-frequency alpha band 4-5 min after the onset of VAB .
	manualset3
231061	6	421580	7	NULL	NULL	0	NULL	 onset 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A low-frequency alpha band appeared immediately after eye closing , but it later disappeared and was replaced by a new development of a high-frequency alpha band 4-5 min after the onset of VAB .
	manualset3
231062	7	421580	7	NULL	NULL	0	NULL	VAB	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A low-frequency alpha band appeared immediately after eye closing , but it later disappeared and was replaced by a new development of a high-frequency alpha band 4-5 min after the onset of VAB .
	manualset3
231138	1	421581	7	NULL	NULL	0	NULL	 cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The cells were cultured for 3 days in an androgen-free medium in the presence of follicle-stimulating hormone ( FSH ) , with or without the specified estrogen .
	manualset3
231139	2	421581	7	NULL	NULL	0	NULL	3 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The cells were cultured for 3 days in an androgen-free medium in the presence of follicle-stimulating hormone ( FSH ) , with or without the specified estrogen .
	manualset3
231141	3	421581	7	NULL	NULL	0	NULL	androgen-free medium	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The cells were cultured for 3 days in an androgen-free medium in the presence of follicle-stimulating hormone ( FSH ) , with or without the specified estrogen .
	manualset3
231142	4	421581	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cells were cultured for 3 days in an androgen-free medium in the presence of follicle-stimulating hormone ( FSH ) , with or without the specified estrogen .
	manualset3
231144	5	421581	7	NULL	NULL	0	NULL	follicle-stimulating hormone ( FSH )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The cells were cultured for 3 days in an androgen-free medium in the presence of follicle-stimulating hormone ( FSH ) , with or without the specified estrogen .
	manualset3
231145	6	421581	7	NULL	NULL	0	NULL	specified estrogen	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The cells were cultured for 3 days in an androgen-free medium in the presence of follicle-stimulating hormone ( FSH ) , with or without the specified estrogen .
	manualset3
231147	1	421582	7	NULL	NULL	0	NULL	paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This paper provides a detailed description of the statistical systems of the U.S. Medicare program and discusses how these data bases can be used for health policy analyses and for international comparisons of health systems at the microeconomic level .
	manualset3
231148	2	421582	7	NULL	NULL	0	NULL	detailed description 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This paper provides a detailed description of the statistical systems of the U.S. Medicare program and discusses how these data bases can be used for health policy analyses and for international comparisons of health systems at the microeconomic level .
	manualset3
231149	3	421582	7	NULL	NULL	0	NULL	statistical systems	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This paper provides a detailed description of the statistical systems of the U.S. Medicare program and discusses how these data bases can be used for health policy analyses and for international comparisons of health systems at the microeconomic level .
	manualset3
231150	4	421582	7	NULL	NULL	0	NULL	U.S. Medicare program	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	This paper provides a detailed description of the statistical systems of the U.S. Medicare program and discusses how these data bases can be used for health policy analyses and for international comparisons of health systems at the microeconomic level .
	manualset3
231151	5	421582	7	NULL	NULL	0	NULL	data bases	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This paper provides a detailed description of the statistical systems of the U.S. Medicare program and discusses how these data bases can be used for health policy analyses and for international comparisons of health systems at the microeconomic level .
	manualset3
231152	6	421582	7	NULL	NULL	0	NULL	health policy analyses	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This paper provides a detailed description of the statistical systems of the U.S. Medicare program and discusses how these data bases can be used for health policy analyses and for international comparisons of health systems at the microeconomic level .
	manualset3
231153	7	421582	7	NULL	NULL	0	NULL	international comparisons	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This paper provides a detailed description of the statistical systems of the U.S. Medicare program and discusses how these data bases can be used for health policy analyses and for international comparisons of health systems at the microeconomic level .
	manualset3
231154	8	421582	7	NULL	NULL	0	NULL	 health systems	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	This paper provides a detailed description of the statistical systems of the U.S. Medicare program and discusses how these data bases can be used for health policy analyses and for international comparisons of health systems at the microeconomic level .
	manualset3
231155	9	421582	7	NULL	NULL	0	NULL	microeconomic level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This paper provides a detailed description of the statistical systems of the U.S. Medicare program and discusses how these data bases can be used for health policy analyses and for international comparisons of health systems at the microeconomic level .
	manualset3
231157	1	421583	7	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In men , the peak GH concentration was also lower in E2 and COR was higher in both bouts than in boys .
	manualset3
231159	2	421583	7	NULL	NULL	0	NULL	peak GH concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In men , the peak GH concentration was also lower in E2 and COR was higher in both bouts than in boys .
	manualset3
231161	3	421583	7	NULL	NULL	0	NULL	E2	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In men , the peak GH concentration was also lower in E2 and COR was higher in both bouts than in boys .
	manualset3
231162	4	421583	7	NULL	NULL	0	NULL	COR	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In men , the peak GH concentration was also lower in E2 and COR was higher in both bouts than in boys .
	manualset3
231163	5	421583	7	NULL	NULL	0	NULL	bouts 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In men , the peak GH concentration was also lower in E2 and COR was higher in both bouts than in boys .
	manualset3
231164	6	421583	7	NULL	NULL	0	NULL	 boys	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In men , the peak GH concentration was also lower in E2 and COR was higher in both bouts than in boys .
	manualset3
231166	1	421584	7	NULL	NULL	0	NULL	10 healthy subjects 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in 10 healthy subjects the effect of chronic enteral supplementation of antioxidants ( vitamins E , C , A , allopurinol , and N-acetylcysteine ) on cytokine production by monocytes at rest , end exercise ( 60-min cycling at 60 % of maximum oxygen consumption ) , and 60 min post-exercise ( recovery ) .
	manualset3
231167	2	421584	7	NULL	NULL	0	NULL	 effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in 10 healthy subjects the effect of chronic enteral supplementation of antioxidants ( vitamins E , C , A , allopurinol , and N-acetylcysteine ) on cytokine production by monocytes at rest , end exercise ( 60-min cycling at 60 % of maximum oxygen consumption ) , and 60 min post-exercise ( recovery ) .
	manualset3
231169	3	421584	7	NULL	NULL	0	NULL	chronic enteral supplementation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in 10 healthy subjects the effect of chronic enteral supplementation of antioxidants ( vitamins E , C , A , allopurinol , and N-acetylcysteine ) on cytokine production by monocytes at rest , end exercise ( 60-min cycling at 60 % of maximum oxygen consumption ) , and 60 min post-exercise ( recovery ) .
	manualset3
231170	4	421584	7	NULL	NULL	0	NULL	antioxidants	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in 10 healthy subjects the effect of chronic enteral supplementation of antioxidants ( vitamins E , C , A , allopurinol , and N-acetylcysteine ) on cytokine production by monocytes at rest , end exercise ( 60-min cycling at 60 % of maximum oxygen consumption ) , and 60 min post-exercise ( recovery ) .
	manualset3
231171	5	421584	7	NULL	NULL	0	NULL	vitamins E	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in 10 healthy subjects the effect of chronic enteral supplementation of antioxidants ( vitamins E , C , A , allopurinol , and N-acetylcysteine ) on cytokine production by monocytes at rest , end exercise ( 60-min cycling at 60 % of maximum oxygen consumption ) , and 60 min post-exercise ( recovery ) .
	manualset3
231172	6	421584	7	NULL	NULL	0	NULL	vitamins C	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in 10 healthy subjects the effect of chronic enteral supplementation of antioxidants ( vitamins E , C , A , allopurinol , and N-acetylcysteine ) on cytokine production by monocytes at rest , end exercise ( 60-min cycling at 60 % of maximum oxygen consumption ) , and 60 min post-exercise ( recovery ) .
	manualset3
231173	7	421584	7	NULL	NULL	0	NULL	vitamins A	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in 10 healthy subjects the effect of chronic enteral supplementation of antioxidants ( vitamins E , C , A , allopurinol , and N-acetylcysteine ) on cytokine production by monocytes at rest , end exercise ( 60-min cycling at 60 % of maximum oxygen consumption ) , and 60 min post-exercise ( recovery ) .
	manualset3
231174	8	421584	7	NULL	NULL	0	NULL	allopurinol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in 10 healthy subjects the effect of chronic enteral supplementation of antioxidants ( vitamins E , C , A , allopurinol , and N-acetylcysteine ) on cytokine production by monocytes at rest , end exercise ( 60-min cycling at 60 % of maximum oxygen consumption ) , and 60 min post-exercise ( recovery ) .
	manualset3
231175	9	421584	7	NULL	NULL	0	NULL	N-acetylcysteine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in 10 healthy subjects the effect of chronic enteral supplementation of antioxidants ( vitamins E , C , A , allopurinol , and N-acetylcysteine ) on cytokine production by monocytes at rest , end exercise ( 60-min cycling at 60 % of maximum oxygen consumption ) , and 60 min post-exercise ( recovery ) .
	manualset3
231176	10	421584	7	NULL	NULL	0	NULL	cytokine production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in 10 healthy subjects the effect of chronic enteral supplementation of antioxidants ( vitamins E , C , A , allopurinol , and N-acetylcysteine ) on cytokine production by monocytes at rest , end exercise ( 60-min cycling at 60 % of maximum oxygen consumption ) , and 60 min post-exercise ( recovery ) .
	manualset3
231177	11	421584	7	NULL	NULL	0	NULL	monocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in 10 healthy subjects the effect of chronic enteral supplementation of antioxidants ( vitamins E , C , A , allopurinol , and N-acetylcysteine ) on cytokine production by monocytes at rest , end exercise ( 60-min cycling at 60 % of maximum oxygen consumption ) , and 60 min post-exercise ( recovery ) .
	manualset3
231178	12	421584	7	NULL	NULL	0	NULL	rest 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in 10 healthy subjects the effect of chronic enteral supplementation of antioxidants ( vitamins E , C , A , allopurinol , and N-acetylcysteine ) on cytokine production by monocytes at rest , end exercise ( 60-min cycling at 60 % of maximum oxygen consumption ) , and 60 min post-exercise ( recovery ) .
	manualset3
231179	13	421584	7	NULL	NULL	0	NULL	 end exercise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in 10 healthy subjects the effect of chronic enteral supplementation of antioxidants ( vitamins E , C , A , allopurinol , and N-acetylcysteine ) on cytokine production by monocytes at rest , end exercise ( 60-min cycling at 60 % of maximum oxygen consumption ) , and 60 min post-exercise ( recovery ) .
	manualset3
231180	14	421584	7	NULL	NULL	0	NULL	 60-min cycling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in 10 healthy subjects the effect of chronic enteral supplementation of antioxidants ( vitamins E , C , A , allopurinol , and N-acetylcysteine ) on cytokine production by monocytes at rest , end exercise ( 60-min cycling at 60 % of maximum oxygen consumption ) , and 60 min post-exercise ( recovery ) .
	manualset3
231181	15	421584	7	NULL	NULL	0	NULL	 60 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in 10 healthy subjects the effect of chronic enteral supplementation of antioxidants ( vitamins E , C , A , allopurinol , and N-acetylcysteine ) on cytokine production by monocytes at rest , end exercise ( 60-min cycling at 60 % of maximum oxygen consumption ) , and 60 min post-exercise ( recovery ) .
	manualset3
231182	16	421584	7	NULL	NULL	0	NULL	maximum oxygen consumption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in 10 healthy subjects the effect of chronic enteral supplementation of antioxidants ( vitamins E , C , A , allopurinol , and N-acetylcysteine ) on cytokine production by monocytes at rest , end exercise ( 60-min cycling at 60 % of maximum oxygen consumption ) , and 60 min post-exercise ( recovery ) .
	manualset3
231183	17	421584	7	NULL	NULL	0	NULL	 60 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in 10 healthy subjects the effect of chronic enteral supplementation of antioxidants ( vitamins E , C , A , allopurinol , and N-acetylcysteine ) on cytokine production by monocytes at rest , end exercise ( 60-min cycling at 60 % of maximum oxygen consumption ) , and 60 min post-exercise ( recovery ) .
	manualset3
231184	18	421584	7	NULL	NULL	0	NULL	post-exercise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in 10 healthy subjects the effect of chronic enteral supplementation of antioxidants ( vitamins E , C , A , allopurinol , and N-acetylcysteine ) on cytokine production by monocytes at rest , end exercise ( 60-min cycling at 60 % of maximum oxygen consumption ) , and 60 min post-exercise ( recovery ) .
	manualset3
231185	19	421584	7	NULL	NULL	0	NULL	recovery 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We studied in 10 healthy subjects the effect of chronic enteral supplementation of antioxidants ( vitamins E , C , A , allopurinol , and N-acetylcysteine ) on cytokine production by monocytes at rest , end exercise ( 60-min cycling at 60 % of maximum oxygen consumption ) , and 60 min post-exercise ( recovery ) .
	manualset3
231186	1	421585	7	NULL	NULL	0	NULL	 dehydrogenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	An altered dehydrogenase in which E261 was replaced by a glutamine was constructed , expressed , purified , and characterized .
	manualset3
231187	2	421585	7	NULL	NULL	0	NULL	E261	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	An altered dehydrogenase in which E261 was replaced by a glutamine was constructed , expressed , purified , and characterized .
	manualset3
231188	3	421585	7	NULL	NULL	0	NULL	glutamine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	An altered dehydrogenase in which E261 was replaced by a glutamine was constructed , expressed , purified , and characterized .
	manualset3
231223	1	421586	7	NULL	NULL	0	NULL	chemotherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	He was treated immediately with chemotherapy .
	manualset3
231224	1	421587	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of basaltic meteorites with variable oxygen isotopic composition suggests the occurrence of multiple basaltic meteorite parent bodies , perhaps similar to 4 Vesta , in the early solar system .
	manualset3
231225	2	421587	7	NULL	NULL	0	NULL	basaltic meteorites 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of basaltic meteorites with variable oxygen isotopic composition suggests the occurrence of multiple basaltic meteorite parent bodies , perhaps similar to 4 Vesta , in the early solar system .
	manualset3
231226	3	421587	7	NULL	NULL	0	NULL	variable oxygen isotopic composition	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of basaltic meteorites with variable oxygen isotopic composition suggests the occurrence of multiple basaltic meteorite parent bodies , perhaps similar to 4 Vesta , in the early solar system .
	manualset3
231227	4	421587	7	NULL	NULL	0	NULL	occurrence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of basaltic meteorites with variable oxygen isotopic composition suggests the occurrence of multiple basaltic meteorite parent bodies , perhaps similar to 4 Vesta , in the early solar system .
	manualset3
231228	5	421587	7	NULL	NULL	0	NULL	 multiple basaltic meteorite parent bodies	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of basaltic meteorites with variable oxygen isotopic composition suggests the occurrence of multiple basaltic meteorite parent bodies , perhaps similar to 4 Vesta , in the early solar system .
	manualset3
231229	6	421587	7	NULL	NULL	0	NULL	4 Vesta 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of basaltic meteorites with variable oxygen isotopic composition suggests the occurrence of multiple basaltic meteorite parent bodies , perhaps similar to 4 Vesta , in the early solar system .
	manualset3
231230	7	421587	7	NULL	NULL	0	NULL	early solar system	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of basaltic meteorites with variable oxygen isotopic composition suggests the occurrence of multiple basaltic meteorite parent bodies , perhaps similar to 4 Vesta , in the early solar system .
	manualset3
231231	1	421588	7	NULL	NULL	0	NULL	business plan	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A business plan is essential to starting a business .
	manualset3
231232	2	421588	7	NULL	NULL	0	NULL	business	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A business plan is essential to starting a business .
	manualset3
231233	1	421589	7	NULL	NULL	0	NULL	Nonspecific reticulo-endothelial uptake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonspecific reticulo-endothelial uptake of radioactivity was a major problem .
	manualset3
231234	2	421589	7	NULL	NULL	NULL	NULL	radioactivity	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nonspecific reticulo-endothelial uptake of radioactivity was a major problem .
	manualset3
231235	3	421589	7	NULL	NULL	0	NULL	major problem	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nonspecific reticulo-endothelial uptake of radioactivity was a major problem .
	manualset3
231236	1	421590	7	NULL	NULL	0	NULL	38	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	38 out of 54 children with congenital toxoplasmosis as well as 34 out of 403 children with congenital human cytomegalovirus disease , with visual/auditory impairment , hospitalized in Infant Department in Children 's Memorial Health Institute between 1995-2001 were enrolled in this study .
	manualset3
231237	2	421590	7	NULL	NULL	0	NULL	 54 children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	38 out of 54 children with congenital toxoplasmosis as well as 34 out of 403 children with congenital human cytomegalovirus disease , with visual/auditory impairment , hospitalized in Infant Department in Children 's Memorial Health Institute between 1995-2001 were enrolled in this study .
	manualset3
231238	3	421590	7	NULL	NULL	0	NULL	congenital toxoplasmosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	38 out of 54 children with congenital toxoplasmosis as well as 34 out of 403 children with congenital human cytomegalovirus disease , with visual/auditory impairment , hospitalized in Infant Department in Children 's Memorial Health Institute between 1995-2001 were enrolled in this study .
	manualset3
231239	4	421590	7	NULL	NULL	0	NULL	34 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	38 out of 54 children with congenital toxoplasmosis as well as 34 out of 403 children with congenital human cytomegalovirus disease , with visual/auditory impairment , hospitalized in Infant Department in Children 's Memorial Health Institute between 1995-2001 were enrolled in this study .
	manualset3
231240	5	421590	7	NULL	NULL	0	NULL	 403 children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	38 out of 54 children with congenital toxoplasmosis as well as 34 out of 403 children with congenital human cytomegalovirus disease , with visual/auditory impairment , hospitalized in Infant Department in Children 's Memorial Health Institute between 1995-2001 were enrolled in this study .
	manualset3
231241	6	421590	7	NULL	NULL	0	NULL	congenital human cytomegalovirus disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	38 out of 54 children with congenital toxoplasmosis as well as 34 out of 403 children with congenital human cytomegalovirus disease , with visual/auditory impairment , hospitalized in Infant Department in Children 's Memorial Health Institute between 1995-2001 were enrolled in this study .
	manualset3
231242	7	421590	7	NULL	NULL	0	NULL	visual/auditory impairment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	38 out of 54 children with congenital toxoplasmosis as well as 34 out of 403 children with congenital human cytomegalovirus disease , with visual/auditory impairment , hospitalized in Infant Department in Children 's Memorial Health Institute between 1995-2001 were enrolled in this study .
	manualset3
231243	8	421590	7	NULL	NULL	0	NULL	Infant Department	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	38 out of 54 children with congenital toxoplasmosis as well as 34 out of 403 children with congenital human cytomegalovirus disease , with visual/auditory impairment , hospitalized in Infant Department in Children 's Memorial Health Institute between 1995-2001 were enrolled in this study .
	manualset3
231244	9	421590	7	NULL	NULL	0	NULL	Children 's Memorial Health Institute	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	38 out of 54 children with congenital toxoplasmosis as well as 34 out of 403 children with congenital human cytomegalovirus disease , with visual/auditory impairment , hospitalized in Infant Department in Children 's Memorial Health Institute between 1995-2001 were enrolled in this study .
	manualset3
231245	10	421590	7	NULL	NULL	0	NULL	1995-2001 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	38 out of 54 children with congenital toxoplasmosis as well as 34 out of 403 children with congenital human cytomegalovirus disease , with visual/auditory impairment , hospitalized in Infant Department in Children 's Memorial Health Institute between 1995-2001 were enrolled in this study .
	manualset3
231246	11	421590	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	38 out of 54 children with congenital toxoplasmosis as well as 34 out of 403 children with congenital human cytomegalovirus disease , with visual/auditory impairment , hospitalized in Infant Department in Children 's Memorial Health Institute between 1995-2001 were enrolled in this study .
	manualset3
231247	1	421591	7	NULL	NULL	0	NULL	Broom ( Sarothamnus scoparius )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Broom ( Sarothamnus scoparius ) poisoning ) .
	manualset3
231248	2	421591	7	NULL	NULL	0	NULL	poisoning 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Broom ( Sarothamnus scoparius ) poisoning ) .
	manualset3
231262	1	421592	7	NULL	NULL	0	NULL	Milder paresis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Milder paresis involved the mimic muscles and the neck extensors .
	manualset3
231263	2	421592	7	NULL	NULL	0	NULL	 muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Milder paresis involved the mimic muscles and the neck extensors .
	manualset3
231264	3	421592	7	NULL	NULL	0	NULL	neck extensors	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Milder paresis involved the mimic muscles and the neck extensors .
	manualset3
231265	1	421593	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of dipyridamole on the metabolism of adenosine were studied in human whole blood .
	manualset3
231266	2	421593	7	NULL	NULL	0	NULL	dipyridamole	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of dipyridamole on the metabolism of adenosine were studied in human whole blood .
	manualset3
231267	3	421593	7	NULL	NULL	0	NULL	metabolism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of dipyridamole on the metabolism of adenosine were studied in human whole blood .
	manualset3
231268	4	421593	7	NULL	NULL	0	NULL	adenosine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of dipyridamole on the metabolism of adenosine were studied in human whole blood .
	manualset3
231269	5	421593	7	NULL	NULL	0	NULL	human whole blood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of dipyridamole on the metabolism of adenosine were studied in human whole blood .
	manualset3
231273	1	421594	7	NULL	NULL	0	NULL	Bullous dermatitis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Bullous dermatitis and bullous pemphigoid .
	manualset3
231274	2	421594	7	NULL	NULL	0	NULL	bullous pemphigoid	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Bullous dermatitis and bullous pemphigoid .
	manualset3
231275	1	421595	7	NULL	NULL	0	NULL	lateralized change detection task	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As in the lateralized change detection task , the number of items on both sides of the display is typically identical , it was not possible to decide between these alternatives yet .
	manualset3
231276	2	421595	7	NULL	NULL	0	NULL	number 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	As in the lateralized change detection task , the number of items on both sides of the display is typically identical , it was not possible to decide between these alternatives yet .
	manualset3
231277	3	421595	7	NULL	NULL	0	NULL	items	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	As in the lateralized change detection task , the number of items on both sides of the display is typically identical , it was not possible to decide between these alternatives yet .
	manualset3
231278	4	421595	7	NULL	NULL	0	NULL	sides of the display	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As in the lateralized change detection task , the number of items on both sides of the display is typically identical , it was not possible to decide between these alternatives yet .
	manualset3
231288	1	421596	7	NULL	NULL	0	NULL	Authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Authors review briefly the pathogenesis , symptoms and treatment of the disease .
	manualset3
231289	2	421596	7	NULL	NULL	0	NULL	pathogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Authors review briefly the pathogenesis , symptoms and treatment of the disease .
	manualset3
231290	3	421596	7	NULL	NULL	0	NULL	 symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Authors review briefly the pathogenesis , symptoms and treatment of the disease .
	manualset3
231291	4	421596	7	NULL	NULL	0	NULL	 treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Authors review briefly the pathogenesis , symptoms and treatment of the disease .
	manualset3
231295	5	421596	7	NULL	NULL	0	NULL	Disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Authors review briefly the pathogenesis , symptoms and treatment of the disease .
	manualset3
231304	1	421597	7	NULL	NULL	NULL	NULL	published results	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Contrary to previously published results no sudden onset of deformation is observed .
	manualset3
231305	2	421597	7	NULL	NULL	0	NULL	sudden onset	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to previously published results no sudden onset of deformation is observed .
	manualset3
231306	3	421597	7	NULL	NULL	0	NULL	deformation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to previously published results no sudden onset of deformation is observed .
	manualset3
231313	1	421598	7	NULL	NULL	0	NULL	 addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the cardiac effects of chloroquine ( CQ ) alone and CQ-CP were compared in 10 age - and sex-matched children .
	manualset3
231314	2	421598	7	NULL	NULL	0	NULL	cardiac effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the cardiac effects of chloroquine ( CQ ) alone and CQ-CP were compared in 10 age - and sex-matched children .
	manualset3
231315	3	421598	7	NULL	NULL	0	NULL	 chloroquine ( CQ )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the cardiac effects of chloroquine ( CQ ) alone and CQ-CP were compared in 10 age - and sex-matched children .
	manualset3
231316	4	421598	7	NULL	NULL	0	NULL	CQ-CP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the cardiac effects of chloroquine ( CQ ) alone and CQ-CP were compared in 10 age - and sex-matched children .
	manualset3
231317	5	421598	7	NULL	NULL	0	NULL	10 age -children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the cardiac effects of chloroquine ( CQ ) alone and CQ-CP were compared in 10 age - and sex-matched children .
	manualset3
231318	6	421598	7	NULL	NULL	0	NULL	sex-matched children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the cardiac effects of chloroquine ( CQ ) alone and CQ-CP were compared in 10 age - and sex-matched children .
	manualset3
231319	1	421599	7	NULL	NULL	0	NULL	Small extracellular injections	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Small extracellular injections of biocytin were made in combination with evoked potential mapping or single-unit analysis and histochemical determination of cortical landmarks .
	manualset3
231320	2	421599	7	NULL	NULL	0	NULL	biocytin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Small extracellular injections of biocytin were made in combination with evoked potential mapping or single-unit analysis and histochemical determination of cortical landmarks .
	manualset3
231321	3	421599	7	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Small extracellular injections of biocytin were made in combination with evoked potential mapping or single-unit analysis and histochemical determination of cortical landmarks .
	manualset3
231322	4	421599	7	NULL	NULL	0	NULL	evoked potential mapping	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Small extracellular injections of biocytin were made in combination with evoked potential mapping or single-unit analysis and histochemical determination of cortical landmarks .
	manualset3
231323	5	421599	7	NULL	NULL	0	NULL	single-unit analysis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Small extracellular injections of biocytin were made in combination with evoked potential mapping or single-unit analysis and histochemical determination of cortical landmarks .
	manualset3
231324	6	421599	7	NULL	NULL	0	NULL	histochemical determination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Small extracellular injections of biocytin were made in combination with evoked potential mapping or single-unit analysis and histochemical determination of cortical landmarks .
	manualset3
231325	7	421599	7	NULL	NULL	0	NULL	cortical landmarks	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Small extracellular injections of biocytin were made in combination with evoked potential mapping or single-unit analysis and histochemical determination of cortical landmarks .
	manualset3
231326	1	421600	7	NULL	NULL	NULL	NULL	increase	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Moreover , the increase in caspase-3 , -8 , and -9 activities in response to StSp was returned to control levels with RBM3 overexpression .
	manualset3
231327	2	421600	7	NULL	NULL	0	NULL	caspase-3 activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the increase in caspase-3 , -8 , and -9 activities in response to StSp was returned to control levels with RBM3 overexpression .
	manualset3
231328	3	421600	7	NULL	NULL	0	NULL	caspase-8 activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the increase in caspase-3 , -8 , and -9 activities in response to StSp was returned to control levels with RBM3 overexpression .
	manualset3
231329	4	421600	7	NULL	NULL	0	NULL	caspase-9 activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the increase in caspase-3 , -8 , and -9 activities in response to StSp was returned to control levels with RBM3 overexpression .
	manualset3
231330	5	421600	7	NULL	NULL	0	NULL	StSp	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the increase in caspase-3 , -8 , and -9 activities in response to StSp was returned to control levels with RBM3 overexpression .
	manualset3
231331	6	421600	7	NULL	NULL	0	NULL	control levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the increase in caspase-3 , -8 , and -9 activities in response to StSp was returned to control levels with RBM3 overexpression .
	manualset3
231332	7	421600	7	NULL	NULL	0	NULL	RBM3 overexpression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the increase in caspase-3 , -8 , and -9 activities in response to StSp was returned to control levels with RBM3 overexpression .
	manualset3
231333	1	421601	7	NULL	NULL	0	NULL	Inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of lymphocyte proliferation by purified macrophages from rat lung .
	manualset3
231334	2	421601	7	NULL	NULL	0	NULL	lymphocyte proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of lymphocyte proliferation by purified macrophages from rat lung .
	manualset3
231335	3	421601	7	NULL	NULL	0	NULL	purified macrophages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of lymphocyte proliferation by purified macrophages from rat lung .
	manualset3
231336	4	421601	7	NULL	NULL	0	NULL	rat lung	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Inhibition of lymphocyte proliferation by purified macrophages from rat lung .
	manualset3
231337	1	421602	7	NULL	NULL	0	NULL	photomirex 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of photomirex and mirex on reproduction in the rat .
	manualset3
231338	2	421602	7	NULL	NULL	0	NULL	mirex	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of photomirex and mirex on reproduction in the rat .
	manualset3
231339	3	421602	7	NULL	NULL	0	NULL	reproduction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of photomirex and mirex on reproduction in the rat .
	manualset3
231340	4	421602	7	NULL	NULL	0	NULL	rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of photomirex and mirex on reproduction in the rat .
	manualset3
231341	1	421603	7	NULL	NULL	0	NULL	Constitutive activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Constitutive activation of Notch signaling is required for the proliferation of a subgroup of human T-cell acute lymphoblastic leukemias ( T-ALL ) .
	manualset3
231342	2	421603	7	NULL	NULL	0	NULL	 proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Constitutive activation of Notch signaling is required for the proliferation of a subgroup of human T-cell acute lymphoblastic leukemias ( T-ALL ) .
	manualset3
231343	3	421603	7	NULL	NULL	0	NULL	subgroup	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Constitutive activation of Notch signaling is required for the proliferation of a subgroup of human T-cell acute lymphoblastic leukemias ( T-ALL ) .
	manualset3
231344	4	421603	7	NULL	NULL	0	NULL	human T-cell acute lymphoblastic leukemias ( T-ALL )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Constitutive activation of Notch signaling is required for the proliferation of a subgroup of human T-cell acute lymphoblastic leukemias ( T-ALL ) .
	manualset3
231345	5	421603	7	NULL	NULL	0	NULL	Notch signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Constitutive activation of Notch signaling is required for the proliferation of a subgroup of human T-cell acute lymphoblastic leukemias ( T-ALL ) .
	manualset3
231346	1	421604	7	NULL	NULL	0	NULL	Treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with both AT-NPD1-SS and AT-NPD1-ME significantly reduced cortical ( by 76 % and 96 % ) , subcortical ( by 61 % and 70 % ) and total ( 69 % and 84 % , respectively ) infarct volumes as defined by histopathology .
	manualset3
231347	2	421604	7	NULL	NULL	0	NULL	AT-NPD1-SS	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with both AT-NPD1-SS and AT-NPD1-ME significantly reduced cortical ( by 76 % and 96 % ) , subcortical ( by 61 % and 70 % ) and total ( 69 % and 84 % , respectively ) infarct volumes as defined by histopathology .
	manualset3
231348	3	421604	7	NULL	NULL	0	NULL	AT-NPD1-ME	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with both AT-NPD1-SS and AT-NPD1-ME significantly reduced cortical ( by 76 % and 96 % ) , subcortical ( by 61 % and 70 % ) and total ( 69 % and 84 % , respectively ) infarct volumes as defined by histopathology .
	manualset3
231349	4	421604	7	NULL	NULL	0	NULL	cortical infarct volumes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with both AT-NPD1-SS and AT-NPD1-ME significantly reduced cortical ( by 76 % and 96 % ) , subcortical ( by 61 % and 70 % ) and total ( 69 % and 84 % , respectively ) infarct volumes as defined by histopathology .
	manualset3
231350	5	421604	7	NULL	NULL	0	NULL	76 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with both AT-NPD1-SS and AT-NPD1-ME significantly reduced cortical ( by 76 % and 96 % ) , subcortical ( by 61 % and 70 % ) and total ( 69 % and 84 % , respectively ) infarct volumes as defined by histopathology .
	manualset3
231351	6	421604	7	NULL	NULL	0	NULL	96 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with both AT-NPD1-SS and AT-NPD1-ME significantly reduced cortical ( by 76 % and 96 % ) , subcortical ( by 61 % and 70 % ) and total ( 69 % and 84 % , respectively ) infarct volumes as defined by histopathology .
	manualset3
231352	7	421604	7	NULL	NULL	0	NULL	subcortical infarct volumes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with both AT-NPD1-SS and AT-NPD1-ME significantly reduced cortical ( by 76 % and 96 % ) , subcortical ( by 61 % and 70 % ) and total ( 69 % and 84 % , respectively ) infarct volumes as defined by histopathology .
	manualset3
231353	8	421604	7	NULL	NULL	0	NULL	61 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with both AT-NPD1-SS and AT-NPD1-ME significantly reduced cortical ( by 76 % and 96 % ) , subcortical ( by 61 % and 70 % ) and total ( 69 % and 84 % , respectively ) infarct volumes as defined by histopathology .
	manualset3
231354	9	421604	7	NULL	NULL	0	NULL	70 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with both AT-NPD1-SS and AT-NPD1-ME significantly reduced cortical ( by 76 % and 96 % ) , subcortical ( by 61 % and 70 % ) and total ( 69 % and 84 % , respectively ) infarct volumes as defined by histopathology .
	manualset3
231355	10	421604	7	NULL	NULL	0	NULL	total infarct volumes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with both AT-NPD1-SS and AT-NPD1-ME significantly reduced cortical ( by 76 % and 96 % ) , subcortical ( by 61 % and 70 % ) and total ( 69 % and 84 % , respectively ) infarct volumes as defined by histopathology .
	manualset3
231356	11	421604	7	NULL	NULL	0	NULL	69 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with both AT-NPD1-SS and AT-NPD1-ME significantly reduced cortical ( by 76 % and 96 % ) , subcortical ( by 61 % and 70 % ) and total ( 69 % and 84 % , respectively ) infarct volumes as defined by histopathology .
	manualset3
231357	12	421604	7	NULL	NULL	0	NULL	84 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with both AT-NPD1-SS and AT-NPD1-ME significantly reduced cortical ( by 76 % and 96 % ) , subcortical ( by 61 % and 70 % ) and total ( 69 % and 84 % , respectively ) infarct volumes as defined by histopathology .
	manualset3
231358	13	421604	7	NULL	NULL	0	NULL	histopathology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with both AT-NPD1-SS and AT-NPD1-ME significantly reduced cortical ( by 76 % and 96 % ) , subcortical ( by 61 % and 70 % ) and total ( 69 % and 84 % , respectively ) infarct volumes as defined by histopathology .
	manualset3
231359	1	421605	7	NULL	NULL	NULL	NULL	Mental hygiene	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Mental hygiene in the college health program .
	manualset3
231360	2	421605	7	NULL	NULL	0	NULL	college health program	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Mental hygiene in the college health program .
	manualset3
231361	1	421606	7	NULL	NULL	0	NULL	pin-site infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We concluded that a pin-site infection that develops during external fixation is a contraindication to the subsequent use of reamed intramedullary nailing in patients who have a fracture of the tibia .
	manualset3
231362	2	421606	7	NULL	NULL	0	NULL	 external fixation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	We concluded that a pin-site infection that develops during external fixation is a contraindication to the subsequent use of reamed intramedullary nailing in patients who have a fracture of the tibia .
	manualset3
231363	3	421606	7	NULL	NULL	0	NULL	contraindication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We concluded that a pin-site infection that develops during external fixation is a contraindication to the subsequent use of reamed intramedullary nailing in patients who have a fracture of the tibia .
	manualset3
231364	4	421606	7	NULL	NULL	0	NULL	subsequent use 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We concluded that a pin-site infection that develops during external fixation is a contraindication to the subsequent use of reamed intramedullary nailing in patients who have a fracture of the tibia .
	manualset3
231365	5	421606	7	NULL	NULL	0	NULL	reamed intramedullary nailing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	We concluded that a pin-site infection that develops during external fixation is a contraindication to the subsequent use of reamed intramedullary nailing in patients who have a fracture of the tibia .
	manualset3
231366	6	421606	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We concluded that a pin-site infection that develops during external fixation is a contraindication to the subsequent use of reamed intramedullary nailing in patients who have a fracture of the tibia .
	manualset3
231367	7	421606	7	NULL	NULL	0	NULL	fracture	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We concluded that a pin-site infection that develops during external fixation is a contraindication to the subsequent use of reamed intramedullary nailing in patients who have a fracture of the tibia .
	manualset3
231368	8	421606	7	NULL	NULL	0	NULL	tibia	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We concluded that a pin-site infection that develops during external fixation is a contraindication to the subsequent use of reamed intramedullary nailing in patients who have a fracture of the tibia .
	manualset3
231369	1	421607	7	NULL	NULL	0	NULL	Therapists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapists think aloud while not looking at their patients ; patients `` overhear '' rather than hear .
	manualset3
231370	2	421607	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapists think aloud while not looking at their patients ; patients `` overhear '' rather than hear .
	manualset3
231371	3	421607	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapists think aloud while not looking at their patients ; patients `` overhear '' rather than hear .
	manualset3
231372	4	421607	7	NULL	NULL	0	NULL	overhear	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapists think aloud while not looking at their patients ; patients `` overhear '' rather than hear .
	manualset3
231373	5	421607	7	NULL	NULL	0	NULL	hear	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Therapists think aloud while not looking at their patients ; patients `` overhear '' rather than hear .
	manualset3
231374	1	421608	7	NULL	NULL	0	NULL	 studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , some studies claim that the upstream lymphoid-primed multipotent progenitor ( LMPP ) is the thymic seeding population , and suggest that CLPs are primarily B-cell-restricted .
	manualset3
231375	2	421608	7	NULL	NULL	0	NULL	lymphoid-primed multipotent progenitor ( LMPP )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , some studies claim that the upstream lymphoid-primed multipotent progenitor ( LMPP ) is the thymic seeding population , and suggest that CLPs are primarily B-cell-restricted .
	manualset3
231376	3	421608	7	NULL	NULL	0	NULL	 thymic seeding population	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , some studies claim that the upstream lymphoid-primed multipotent progenitor ( LMPP ) is the thymic seeding population , and suggest that CLPs are primarily B-cell-restricted .
	manualset3
231377	4	421608	7	NULL	NULL	0	NULL	CLPs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	However , some studies claim that the upstream lymphoid-primed multipotent progenitor ( LMPP ) is the thymic seeding population , and suggest that CLPs are primarily B-cell-restricted .
	manualset3
231378	1	421609	7	NULL	NULL	0	NULL	Development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Development of the new surgical fiberoptic nephro-ureteroscope ) .
	manualset3
231379	2	421609	7	NULL	NULL	0	NULL	new surgical fiberoptic nephro-ureteroscope 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	( Development of the new surgical fiberoptic nephro-ureteroscope ) .
	manualset3
231380	1	421610	7	NULL	NULL	0	NULL	process model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	An alternative is to use a process model of reduced order for on-line inference of state variables based on secondary process measurements , e.g. pH and redox potential .
	manualset3
231381	2	421610	7	NULL	NULL	0	NULL	reduced order	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An alternative is to use a process model of reduced order for on-line inference of state variables based on secondary process measurements , e.g. pH and redox potential .
	manualset3
231382	3	421610	7	NULL	NULL	0	NULL	on-line inference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An alternative is to use a process model of reduced order for on-line inference of state variables based on secondary process measurements , e.g. pH and redox potential .
	manualset3
231383	4	421610	7	NULL	NULL	0	NULL	state variables	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	An alternative is to use a process model of reduced order for on-line inference of state variables based on secondary process measurements , e.g. pH and redox potential .
	manualset3
231384	5	421610	7	NULL	NULL	0	NULL	secondary process measurements	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An alternative is to use a process model of reduced order for on-line inference of state variables based on secondary process measurements , e.g. pH and redox potential .
	manualset3
231385	6	421610	7	NULL	NULL	0	NULL	 pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An alternative is to use a process model of reduced order for on-line inference of state variables based on secondary process measurements , e.g. pH and redox potential .
	manualset3
231386	7	421610	7	NULL	NULL	0	NULL	redox potential	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An alternative is to use a process model of reduced order for on-line inference of state variables based on secondary process measurements , e.g. pH and redox potential .
	manualset3
231387	1	421611	7	NULL	NULL	0	NULL	NA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The NA of the 're - emerged ' virus A/USSR/92 / 77 ( H1N1 ) was antigenically related but not identical to influenza A viruses isolated in 1949 ( A/Paris/49 ( H1N1 ) , A/Geneva/49 ( H1N1 ) which thus predates the previously observed antigenic similarity of A/USSR/77 with A/FW/50 ( H1N1 ) virus .
	manualset3
231388	2	421611	7	NULL	NULL	0	NULL	're - emerged ' virus A/USSR/92 / 77 ( H1N1 )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The NA of the 're - emerged ' virus A/USSR/92 / 77 ( H1N1 ) was antigenically related but not identical to influenza A viruses isolated in 1949 ( A/Paris/49 ( H1N1 ) , A/Geneva/49 ( H1N1 ) which thus predates the previously observed antigenic similarity of A/USSR/77 with A/FW/50 ( H1N1 ) virus .
	manualset3
231389	3	421611	7	NULL	NULL	0	NULL	influenza A viruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The NA of the 're - emerged ' virus A/USSR/92 / 77 ( H1N1 ) was antigenically related but not identical to influenza A viruses isolated in 1949 ( A/Paris/49 ( H1N1 ) , A/Geneva/49 ( H1N1 ) which thus predates the previously observed antigenic similarity of A/USSR/77 with A/FW/50 ( H1N1 ) virus .
	manualset3
231390	4	421611	7	NULL	NULL	0	NULL	1949	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	The NA of the 're - emerged ' virus A/USSR/92 / 77 ( H1N1 ) was antigenically related but not identical to influenza A viruses isolated in 1949 ( A/Paris/49 ( H1N1 ) , A/Geneva/49 ( H1N1 ) which thus predates the previously observed antigenic similarity of A/USSR/77 with A/FW/50 ( H1N1 ) virus .
	manualset3
231391	5	421611	7	NULL	NULL	0	NULL	( A/Paris/49 ( H1N1 )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The NA of the 're - emerged ' virus A/USSR/92 / 77 ( H1N1 ) was antigenically related but not identical to influenza A viruses isolated in 1949 ( A/Paris/49 ( H1N1 ) , A/Geneva/49 ( H1N1 ) which thus predates the previously observed antigenic similarity of A/USSR/77 with A/FW/50 ( H1N1 ) virus .
	manualset3
231392	6	421611	7	NULL	NULL	0	NULL	A/Geneva/49 ( H1N1 ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The NA of the 're - emerged ' virus A/USSR/92 / 77 ( H1N1 ) was antigenically related but not identical to influenza A viruses isolated in 1949 ( A/Paris/49 ( H1N1 ) , A/Geneva/49 ( H1N1 ) which thus predates the previously observed antigenic similarity of A/USSR/77 with A/FW/50 ( H1N1 ) virus .
	manualset3
231393	7	421611	7	NULL	NULL	0	NULL	antigenic similarity	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The NA of the 're - emerged ' virus A/USSR/92 / 77 ( H1N1 ) was antigenically related but not identical to influenza A viruses isolated in 1949 ( A/Paris/49 ( H1N1 ) , A/Geneva/49 ( H1N1 ) which thus predates the previously observed antigenic similarity of A/USSR/77 with A/FW/50 ( H1N1 ) virus .
	manualset3
231394	8	421611	7	NULL	NULL	0	NULL	A/USSR/77 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The NA of the 're - emerged ' virus A/USSR/92 / 77 ( H1N1 ) was antigenically related but not identical to influenza A viruses isolated in 1949 ( A/Paris/49 ( H1N1 ) , A/Geneva/49 ( H1N1 ) which thus predates the previously observed antigenic similarity of A/USSR/77 with A/FW/50 ( H1N1 ) virus .
	manualset3
231395	9	421611	7	NULL	NULL	0	NULL	A/FW/50 ( H1N1 ) virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The NA of the 're - emerged ' virus A/USSR/92 / 77 ( H1N1 ) was antigenically related but not identical to influenza A viruses isolated in 1949 ( A/Paris/49 ( H1N1 ) , A/Geneva/49 ( H1N1 ) which thus predates the previously observed antigenic similarity of A/USSR/77 with A/FW/50 ( H1N1 ) virus .
	manualset3
231396	1	421612	7	NULL	NULL	0	NULL	Characterization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Characterization of angiotensin II receptors in smooth muscle preparations of the guinea pig in vitro .
	manualset3
231397	2	421612	7	NULL	NULL	NULL	NULL	angiotensin II receptors	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Characterization of angiotensin II receptors in smooth muscle preparations of the guinea pig in vitro .
	manualset3
231398	3	421612	7	NULL	NULL	0	NULL	smooth muscle preparations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Characterization of angiotensin II receptors in smooth muscle preparations of the guinea pig in vitro .
	manualset3
231399	4	421612	7	NULL	NULL	0	NULL	guinea pig 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Characterization of angiotensin II receptors in smooth muscle preparations of the guinea pig in vitro .
	manualset3
231400	1	421613	7	NULL	NULL	0	NULL	egg-transmitted poultry diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Most exotic and egg-transmitted poultry diseases have been controlled by reduction or eradication policies .
	manualset3
231401	2	421613	7	NULL	NULL	0	NULL	reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most exotic and egg-transmitted poultry diseases have been controlled by reduction or eradication policies .
	manualset3
231402	3	421613	7	NULL	NULL	0	NULL	eradication policies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Most exotic and egg-transmitted poultry diseases have been controlled by reduction or eradication policies .
	manualset3
231403	1	421614	7	NULL	NULL	0	NULL	 novel process configuration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel process configuration that achieves both carbon and nitrogen removal using MFC is designed and demonstrated .
	manualset3
231404	2	421614	7	NULL	NULL	0	NULL	carbon removal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel process configuration that achieves both carbon and nitrogen removal using MFC is designed and demonstrated .
	manualset3
231405	3	421614	7	NULL	NULL	0	NULL	 nitrogen removal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel process configuration that achieves both carbon and nitrogen removal using MFC is designed and demonstrated .
	manualset3
231406	4	421614	7	NULL	NULL	0	NULL	MFC 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	A novel process configuration that achieves both carbon and nitrogen removal using MFC is designed and demonstrated .
	manualset3
231407	1	421615	7	NULL	NULL	0	NULL	ELISA probes	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	ELISA probes showed that the monoclonal antibodies recognized different , nonoverlapping , unrepeated , proteinaceous epitopes present in the same compounds of bovine Reissner 's fiber .
	manualset3
231408	2	421615	7	NULL	NULL	0	NULL	monoclonal antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	ELISA probes showed that the monoclonal antibodies recognized different , nonoverlapping , unrepeated , proteinaceous epitopes present in the same compounds of bovine Reissner 's fiber .
	manualset3
231409	3	421615	7	NULL	NULL	NULL	NULL	compounds	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ELISA probes showed that the monoclonal antibodies recognized different , nonoverlapping , unrepeated , proteinaceous epitopes present in the same compounds of bovine Reissner 's fiber .
	manualset3
231410	4	421615	7	NULL	NULL	0	NULL	bovine Reissner 's fiber 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	ELISA probes showed that the monoclonal antibodies recognized different , nonoverlapping , unrepeated , proteinaceous epitopes present in the same compounds of bovine Reissner 's fiber .
	manualset3
233227	5	421615	7	NULL	NULL	0	NULL	proteinaceous epitopes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	ELISA probes showed that the monoclonal antibodies recognized different , nonoverlapping , unrepeated , proteinaceous epitopes present in the same compounds of bovine Reissner 's fiber .
	manualset3
231411	1	421616	7	NULL	NULL	0	NULL	 purified enzyme	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The purified enzyme had a specific activity of 75 mumol min-1 mg-1 .
	manualset3
231412	2	421616	7	NULL	NULL	0	NULL	 specific activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purified enzyme had a specific activity of 75 mumol min-1 mg-1 .
	manualset3
231413	3	421616	7	NULL	NULL	0	NULL	75 mumol min-1 mg-1	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purified enzyme had a specific activity of 75 mumol min-1 mg-1 .
	manualset3
231414	1	421617	7	NULL	NULL	0	NULL	evolutionary epidemiological mechanism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An evolutionary epidemiological mechanism , with applications to type A influenza .
	manualset3
231415	2	421617	7	NULL	NULL	0	NULL	applications 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An evolutionary epidemiological mechanism , with applications to type A influenza .
	manualset3
231416	3	421617	7	NULL	NULL	0	NULL	type A influenza	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	An evolutionary epidemiological mechanism , with applications to type A influenza .
	manualset3
231419	1	421618	7	NULL	NULL	0	NULL	Hypertensive cardiovascular disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypertensive cardiovascular disease ; nature and pathogenesis of the arteriolar sclerosis induced by bilateral nephrectomy as revealed by a study of its tinctorial characteristics .
	manualset3
231420	2	421618	7	NULL	NULL	0	NULL	nature	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypertensive cardiovascular disease ; nature and pathogenesis of the arteriolar sclerosis induced by bilateral nephrectomy as revealed by a study of its tinctorial characteristics .
	manualset3
231421	3	421618	7	NULL	NULL	0	NULL	pathogenesis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypertensive cardiovascular disease ; nature and pathogenesis of the arteriolar sclerosis induced by bilateral nephrectomy as revealed by a study of its tinctorial characteristics .
	manualset3
231422	4	421618	7	NULL	NULL	0	NULL	 arteriolar sclerosis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypertensive cardiovascular disease ; nature and pathogenesis of the arteriolar sclerosis induced by bilateral nephrectomy as revealed by a study of its tinctorial characteristics .
	manualset3
231423	5	421618	7	NULL	NULL	0	NULL	bilateral nephrectomy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypertensive cardiovascular disease ; nature and pathogenesis of the arteriolar sclerosis induced by bilateral nephrectomy as revealed by a study of its tinctorial characteristics .
	manualset3
231424	6	421618	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypertensive cardiovascular disease ; nature and pathogenesis of the arteriolar sclerosis induced by bilateral nephrectomy as revealed by a study of its tinctorial characteristics .
	manualset3
231425	7	421618	7	NULL	NULL	0	NULL	tinctorial characteristics .	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypertensive cardiovascular disease ; nature and pathogenesis of the arteriolar sclerosis induced by bilateral nephrectomy as revealed by a study of its tinctorial characteristics .
	manualset3
231426	1	421619	7	NULL	NULL	0	NULL	Conjoined twins	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conjoined twins were diagnosed at 10 weeks of gestation in a triplet pregnancy obtained by means of in vitro fertilization .
	manualset3
231427	2	421619	7	NULL	NULL	0	NULL	10 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Conjoined twins were diagnosed at 10 weeks of gestation in a triplet pregnancy obtained by means of in vitro fertilization .
	manualset3
231428	3	421619	7	NULL	NULL	0	NULL	gestation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Conjoined twins were diagnosed at 10 weeks of gestation in a triplet pregnancy obtained by means of in vitro fertilization .
	manualset3
231429	4	421619	7	NULL	NULL	0	NULL	triplet pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conjoined twins were diagnosed at 10 weeks of gestation in a triplet pregnancy obtained by means of in vitro fertilization .
	manualset3
231430	5	421619	7	NULL	NULL	0	NULL	in vitro fertilization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Conjoined twins were diagnosed at 10 weeks of gestation in a triplet pregnancy obtained by means of in vitro fertilization .
	manualset3
231431	1	421620	7	NULL	NULL	0	NULL	analogous pattern	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An analogous pattern of O-dealkylation has been reported in mammalian systems .
	manualset3
231432	2	421620	7	NULL	NULL	0	NULL	O-dealkylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An analogous pattern of O-dealkylation has been reported in mammalian systems .
	manualset3
231433	3	421620	7	NULL	NULL	0	NULL	mammalian systems	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	An analogous pattern of O-dealkylation has been reported in mammalian systems .
	manualset3
231434	1	421621	7	NULL	NULL	0	NULL	proposed techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the proposed techniques are useful in both the bright-field and the fluorescence modes and for reflection and transmission geometries .
	manualset3
231435	2	421621	7	NULL	NULL	0	NULL	bright-field	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the proposed techniques are useful in both the bright-field and the fluorescence modes and for reflection and transmission geometries .
	manualset3
231436	3	421621	7	NULL	NULL	0	NULL	fluorescence modes	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the proposed techniques are useful in both the bright-field and the fluorescence modes and for reflection and transmission geometries .
	manualset3
231437	4	421621	7	NULL	NULL	0	NULL	reflection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the proposed techniques are useful in both the bright-field and the fluorescence modes and for reflection and transmission geometries .
	manualset3
231438	5	421621	7	NULL	NULL	0	NULL	 transmission geometries	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is shown that the proposed techniques are useful in both the bright-field and the fluorescence modes and for reflection and transmission geometries .
	manualset3
231439	1	421622	7	NULL	NULL	0	NULL	28 other cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 28 other cases , however , the egg displayed a slow increase in ( Ca2 + ) i of 0.15 microM , starting around 15 minutes after fertilization and reaching a plateau level around 10 minutes later .
	manualset3
231440	2	421622	7	NULL	NULL	0	NULL	egg	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In 28 other cases , however , the egg displayed a slow increase in ( Ca2 + ) i of 0.15 microM , starting around 15 minutes after fertilization and reaching a plateau level around 10 minutes later .
	manualset3
231441	3	421622	7	NULL	NULL	0	NULL	slow increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In 28 other cases , however , the egg displayed a slow increase in ( Ca2 + ) i of 0.15 microM , starting around 15 minutes after fertilization and reaching a plateau level around 10 minutes later .
	manualset3
231442	4	421622	7	NULL	NULL	0	NULL	Ca2 +	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In 28 other cases , however , the egg displayed a slow increase in ( Ca2 + ) i of 0.15 microM , starting around 15 minutes after fertilization and reaching a plateau level around 10 minutes later .
	manualset3
231443	5	421622	7	NULL	NULL	0	NULL	 0.15 microM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 28 other cases , however , the egg displayed a slow increase in ( Ca2 + ) i of 0.15 microM , starting around 15 minutes after fertilization and reaching a plateau level around 10 minutes later .
	manualset3
231444	6	421622	7	NULL	NULL	0	NULL	15 minutes	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In 28 other cases , however , the egg displayed a slow increase in ( Ca2 + ) i of 0.15 microM , starting around 15 minutes after fertilization and reaching a plateau level around 10 minutes later .
	manualset3
231445	7	421622	7	NULL	NULL	0	NULL	 fertilization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In 28 other cases , however , the egg displayed a slow increase in ( Ca2 + ) i of 0.15 microM , starting around 15 minutes after fertilization and reaching a plateau level around 10 minutes later .
	manualset3
231446	8	421622	7	NULL	NULL	0	NULL	plateau level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 28 other cases , however , the egg displayed a slow increase in ( Ca2 + ) i of 0.15 microM , starting around 15 minutes after fertilization and reaching a plateau level around 10 minutes later .
	manualset3
231447	9	421622	7	NULL	NULL	0	NULL	10 minutes	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In 28 other cases , however , the egg displayed a slow increase in ( Ca2 + ) i of 0.15 microM , starting around 15 minutes after fertilization and reaching a plateau level around 10 minutes later .
	manualset3
231448	1	421623	7	NULL	NULL	0	NULL	Ultrastructural studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural studies which indicate two types of glial cells in the subependymal plate contradicted by the results of the present investigation demonstrating one type of glial cells in the hypothalamic subependymal plate .
	manualset3
231449	2	421623	7	NULL	NULL	0	NULL	two types	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural studies which indicate two types of glial cells in the subependymal plate contradicted by the results of the present investigation demonstrating one type of glial cells in the hypothalamic subependymal plate .
	manualset3
231450	3	421623	7	NULL	NULL	0	NULL	glial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural studies which indicate two types of glial cells in the subependymal plate contradicted by the results of the present investigation demonstrating one type of glial cells in the hypothalamic subependymal plate .
	manualset3
231451	4	421623	7	NULL	NULL	0	NULL	 subependymal plate 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural studies which indicate two types of glial cells in the subependymal plate contradicted by the results of the present investigation demonstrating one type of glial cells in the hypothalamic subependymal plate .
	manualset3
231452	5	421623	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural studies which indicate two types of glial cells in the subependymal plate contradicted by the results of the present investigation demonstrating one type of glial cells in the hypothalamic subependymal plate .
	manualset3
231453	6	421623	7	NULL	NULL	0	NULL	present investigation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural studies which indicate two types of glial cells in the subependymal plate contradicted by the results of the present investigation demonstrating one type of glial cells in the hypothalamic subependymal plate .
	manualset3
231454	7	421623	7	NULL	NULL	0	NULL	 one type	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural studies which indicate two types of glial cells in the subependymal plate contradicted by the results of the present investigation demonstrating one type of glial cells in the hypothalamic subependymal plate .
	manualset3
231455	8	421623	7	NULL	NULL	0	NULL	glial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural studies which indicate two types of glial cells in the subependymal plate contradicted by the results of the present investigation demonstrating one type of glial cells in the hypothalamic subependymal plate .
	manualset3
231456	9	421623	7	NULL	NULL	0	NULL	hypothalamic subependymal plate	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrastructural studies which indicate two types of glial cells in the subependymal plate contradicted by the results of the present investigation demonstrating one type of glial cells in the hypothalamic subependymal plate .
	manualset3
231457	1	421624	7	NULL	NULL	0	NULL	prolactin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , prolactin has an antidiuretic effect similar to that which occurs as a result of ADH action on the kidney and does not require either the release or the presence of ADH in order to cause the antidiuresis .
	manualset3
231458	2	421624	7	NULL	NULL	0	NULL	 antidiuretic effect 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , prolactin has an antidiuretic effect similar to that which occurs as a result of ADH action on the kidney and does not require either the release or the presence of ADH in order to cause the antidiuresis .
	manualset3
231459	3	421624	7	NULL	NULL	0	NULL	result	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , prolactin has an antidiuretic effect similar to that which occurs as a result of ADH action on the kidney and does not require either the release or the presence of ADH in order to cause the antidiuresis .
	manualset3
231460	4	421624	7	NULL	NULL	0	NULL	ADH action	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , prolactin has an antidiuretic effect similar to that which occurs as a result of ADH action on the kidney and does not require either the release or the presence of ADH in order to cause the antidiuresis .
	manualset3
231461	5	421624	7	NULL	NULL	0	NULL	kidney	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , prolactin has an antidiuretic effect similar to that which occurs as a result of ADH action on the kidney and does not require either the release or the presence of ADH in order to cause the antidiuresis .
	manualset3
231462	6	421624	7	NULL	NULL	0	NULL	release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , prolactin has an antidiuretic effect similar to that which occurs as a result of ADH action on the kidney and does not require either the release or the presence of ADH in order to cause the antidiuresis .
	manualset3
231463	7	421624	7	NULL	NULL	0	NULL	 presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , prolactin has an antidiuretic effect similar to that which occurs as a result of ADH action on the kidney and does not require either the release or the presence of ADH in order to cause the antidiuresis .
	manualset3
231464	8	421624	7	NULL	NULL	0	NULL	ADH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , prolactin has an antidiuretic effect similar to that which occurs as a result of ADH action on the kidney and does not require either the release or the presence of ADH in order to cause the antidiuresis .
	manualset3
231465	9	421624	7	NULL	NULL	0	NULL	antidiuresis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , prolactin has an antidiuretic effect similar to that which occurs as a result of ADH action on the kidney and does not require either the release or the presence of ADH in order to cause the antidiuresis .
	manualset3
231466	1	421625	7	NULL	NULL	0	NULL	LC50 estimates 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Average LC50 estimates for selected lotic invertebrates , based on a one hour dosing regime , were : 2.71 mg/L for Simulium vittatum , 4.59 mg/L for Hydropsyche spp. , and 13.41 mg/L for Isonychia bicolor .
	manualset3
231467	2	421625	7	NULL	NULL	0	NULL	lotic invertebrates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Average LC50 estimates for selected lotic invertebrates , based on a one hour dosing regime , were : 2.71 mg/L for Simulium vittatum , 4.59 mg/L for Hydropsyche spp. , and 13.41 mg/L for Isonychia bicolor .
	manualset3
231468	3	421625	7	NULL	NULL	0	NULL	one hour dosing regime	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Average LC50 estimates for selected lotic invertebrates , based on a one hour dosing regime , were : 2.71 mg/L for Simulium vittatum , 4.59 mg/L for Hydropsyche spp. , and 13.41 mg/L for Isonychia bicolor .
	manualset3
231469	4	421625	7	NULL	NULL	0	NULL	2.71 mg/L	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Average LC50 estimates for selected lotic invertebrates , based on a one hour dosing regime , were : 2.71 mg/L for Simulium vittatum , 4.59 mg/L for Hydropsyche spp. , and 13.41 mg/L for Isonychia bicolor .
	manualset3
231470	5	421625	7	NULL	NULL	0	NULL	Simulium vittatum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Average LC50 estimates for selected lotic invertebrates , based on a one hour dosing regime , were : 2.71 mg/L for Simulium vittatum , 4.59 mg/L for Hydropsyche spp. , and 13.41 mg/L for Isonychia bicolor .
	manualset3
231471	6	421625	7	NULL	NULL	0	NULL	4.59 mg/L 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Average LC50 estimates for selected lotic invertebrates , based on a one hour dosing regime , were : 2.71 mg/L for Simulium vittatum , 4.59 mg/L for Hydropsyche spp. , and 13.41 mg/L for Isonychia bicolor .
	manualset3
231472	7	421625	7	NULL	NULL	0	NULL	Hydropsyche spp. 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Average LC50 estimates for selected lotic invertebrates , based on a one hour dosing regime , were : 2.71 mg/L for Simulium vittatum , 4.59 mg/L for Hydropsyche spp. , and 13.41 mg/L for Isonychia bicolor .
	manualset3
231473	8	421625	7	NULL	NULL	0	NULL	13.41 mg/L	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Average LC50 estimates for selected lotic invertebrates , based on a one hour dosing regime , were : 2.71 mg/L for Simulium vittatum , 4.59 mg/L for Hydropsyche spp. , and 13.41 mg/L for Isonychia bicolor .
	manualset3
231474	9	421625	7	NULL	NULL	0	NULL	Isonychia bicolor	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Average LC50 estimates for selected lotic invertebrates , based on a one hour dosing regime , were : 2.71 mg/L for Simulium vittatum , 4.59 mg/L for Hydropsyche spp. , and 13.41 mg/L for Isonychia bicolor .
	manualset3
231475	1	421626	7	NULL	NULL	0	NULL	Noggin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Noggin recruits mesoderm progenitors from the dorsal aorta to a skeletal myogenic fate .
	manualset3
231476	2	421626	7	NULL	NULL	0	NULL	mesoderm progenitors	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Noggin recruits mesoderm progenitors from the dorsal aorta to a skeletal myogenic fate .
	manualset3
231477	3	421626	7	NULL	NULL	0	NULL	dorsal aorta 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Noggin recruits mesoderm progenitors from the dorsal aorta to a skeletal myogenic fate .
	manualset3
231478	4	421626	7	NULL	NULL	0	NULL	skeletal myogenic fate	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Noggin recruits mesoderm progenitors from the dorsal aorta to a skeletal myogenic fate .
	manualset3
231479	1	421627	7	NULL	NULL	0	NULL	glutathione reductase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the glutathione reductase activity was significantly increased , whereas the glutathione peroxidase was decreased .
	manualset3
231480	2	421627	7	NULL	NULL	0	NULL	glutathione peroxidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , the glutathione reductase activity was significantly increased , whereas the glutathione peroxidase was decreased .
	manualset3
231481	1	421628	7	NULL	NULL	0	NULL	GPIb	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We have recently shown that GPIb on platelets is cleaved by metalloproteinase-dependent mechanisms in response to mitochondrial injury .
	manualset3
231482	2	421628	7	NULL	NULL	0	NULL	metalloproteinase-dependent mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We have recently shown that GPIb on platelets is cleaved by metalloproteinase-dependent mechanisms in response to mitochondrial injury .
	manualset3
231483	3	421628	7	NULL	NULL	0	NULL	mitochondrial injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We have recently shown that GPIb on platelets is cleaved by metalloproteinase-dependent mechanisms in response to mitochondrial injury .
	manualset3
233228	4	421628	7	NULL	NULL	0	NULL	 platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We have recently shown that GPIb on platelets is cleaved by metalloproteinase-dependent mechanisms in response to mitochondrial injury .
	manualset3
231484	1	421629	7	NULL	NULL	0	NULL	Rice exonuclease-1 homolog	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Rice exonuclease-1 homolog , OsEXO1 , that interacts with DNA polymerase lambda and RPA subunit proteins , is involved in cell proliferation .
	manualset3
231485	2	421629	7	NULL	NULL	0	NULL	OsEXO1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Rice exonuclease-1 homolog , OsEXO1 , that interacts with DNA polymerase lambda and RPA subunit proteins , is involved in cell proliferation .
	manualset3
231486	3	421629	7	NULL	NULL	0	NULL	DNA polymerase lambda 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Rice exonuclease-1 homolog , OsEXO1 , that interacts with DNA polymerase lambda and RPA subunit proteins , is involved in cell proliferation .
	manualset3
231487	4	421629	7	NULL	NULL	0	NULL	RPA subunit proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Rice exonuclease-1 homolog , OsEXO1 , that interacts with DNA polymerase lambda and RPA subunit proteins , is involved in cell proliferation .
	manualset3
231488	5	421629	7	NULL	NULL	0	NULL	 cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Rice exonuclease-1 homolog , OsEXO1 , that interacts with DNA polymerase lambda and RPA subunit proteins , is involved in cell proliferation .
	manualset3
231489	1	421630	7	NULL	NULL	0	NULL	poly ( I : C ) stimulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that poly ( I : C ) stimulation induces selective autophagic degradation of the TLR adaptor molecule TRIF and the signaling molecule TRAF6 , which is revealed by gene silencing of the ubiquitin-editing enzyme A20 .
	manualset3
231490	2	421630	7	NULL	NULL	0	NULL	selective autophagic degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that poly ( I : C ) stimulation induces selective autophagic degradation of the TLR adaptor molecule TRIF and the signaling molecule TRAF6 , which is revealed by gene silencing of the ubiquitin-editing enzyme A20 .
	manualset3
231491	3	421630	7	NULL	NULL	0	NULL	TLR adaptor molecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that poly ( I : C ) stimulation induces selective autophagic degradation of the TLR adaptor molecule TRIF and the signaling molecule TRAF6 , which is revealed by gene silencing of the ubiquitin-editing enzyme A20 .
	manualset3
231492	4	421630	7	NULL	NULL	0	NULL	TRIF 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that poly ( I : C ) stimulation induces selective autophagic degradation of the TLR adaptor molecule TRIF and the signaling molecule TRAF6 , which is revealed by gene silencing of the ubiquitin-editing enzyme A20 .
	manualset3
231493	5	421630	7	NULL	NULL	0	NULL	signaling molecule 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that poly ( I : C ) stimulation induces selective autophagic degradation of the TLR adaptor molecule TRIF and the signaling molecule TRAF6 , which is revealed by gene silencing of the ubiquitin-editing enzyme A20 .
	manualset3
231494	6	421630	7	NULL	NULL	0	NULL	TRAF6 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that poly ( I : C ) stimulation induces selective autophagic degradation of the TLR adaptor molecule TRIF and the signaling molecule TRAF6 , which is revealed by gene silencing of the ubiquitin-editing enzyme A20 .
	manualset3
231495	7	421630	7	NULL	NULL	0	NULL	gene silencing	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that poly ( I : C ) stimulation induces selective autophagic degradation of the TLR adaptor molecule TRIF and the signaling molecule TRAF6 , which is revealed by gene silencing of the ubiquitin-editing enzyme A20 .
	manualset3
231496	8	421630	7	NULL	NULL	0	NULL	ubiquitin-editing enzyme A20	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we report that poly ( I : C ) stimulation induces selective autophagic degradation of the TLR adaptor molecule TRIF and the signaling molecule TRAF6 , which is revealed by gene silencing of the ubiquitin-editing enzyme A20 .
	manualset3
231497	1	421631	7	NULL	NULL	0	NULL	mutant enzyme	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The mutant enzyme was also activated more by ATP and inhibited less by CTP as compared to the wild-type enzyme .
	manualset3
231498	2	421631	7	NULL	NULL	0	NULL	ATP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The mutant enzyme was also activated more by ATP and inhibited less by CTP as compared to the wild-type enzyme .
	manualset3
231499	3	421631	7	NULL	NULL	0	NULL	CTP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The mutant enzyme was also activated more by ATP and inhibited less by CTP as compared to the wild-type enzyme .
	manualset3
231500	4	421631	7	NULL	NULL	0	NULL	wild-type enzyme 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The mutant enzyme was also activated more by ATP and inhibited less by CTP as compared to the wild-type enzyme .
	manualset3
231501	1	421632	7	NULL	NULL	0	NULL	neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	These neurons have multiterminal receptive fields and respond phaso-tonically to cuticular distortion .
	manualset3
231502	2	421632	7	NULL	NULL	0	NULL	multiterminal receptive fields 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These neurons have multiterminal receptive fields and respond phaso-tonically to cuticular distortion .
	manualset3
231503	3	421632	7	NULL	NULL	0	NULL	cuticular distortion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These neurons have multiterminal receptive fields and respond phaso-tonically to cuticular distortion .
	manualset3
231504	1	421633	7	NULL	NULL	0	NULL	 analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An analysis of 653 trials of penile vibratory stimulation in men with spinal cord injury .
	manualset3
231505	2	421633	7	NULL	NULL	0	NULL	653 trials 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An analysis of 653 trials of penile vibratory stimulation in men with spinal cord injury .
	manualset3
231506	3	421633	7	NULL	NULL	0	NULL	penile vibratory stimulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An analysis of 653 trials of penile vibratory stimulation in men with spinal cord injury .
	manualset3
231507	4	421633	7	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	An analysis of 653 trials of penile vibratory stimulation in men with spinal cord injury .
	manualset3
231508	5	421633	7	NULL	NULL	0	NULL	spinal cord injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An analysis of 653 trials of penile vibratory stimulation in men with spinal cord injury .
	manualset3
231707	1	421634	7	NULL	NULL	0	NULL	Red	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Red from KA1 was crystallized at 278 K by the hanging-drop vapour-diffusion method using PEG 4000 .
	manualset3
231708	2	421634	7	NULL	NULL	0	NULL	KA1 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Red from KA1 was crystallized at 278 K by the hanging-drop vapour-diffusion method using PEG 4000 .
	manualset3
231709	3	421634	7	NULL	NULL	0	NULL	 278 K	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Red from KA1 was crystallized at 278 K by the hanging-drop vapour-diffusion method using PEG 4000 .
	manualset3
231710	4	421634	7	NULL	NULL	NULL	NULL	hanging-drop vapour-diffusion method	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Red from KA1 was crystallized at 278 K by the hanging-drop vapour-diffusion method using PEG 4000 .
	manualset3
231711	5	421634	7	NULL	NULL	0	NULL	PEG 4000	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Red from KA1 was crystallized at 278 K by the hanging-drop vapour-diffusion method using PEG 4000 .
	manualset3
231712	1	421635	7	NULL	NULL	0	NULL	transgenic mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In transgenic mice bearing Epo-TAg at homologous and heterologous insertion sites , renal expression was restricted to a population of cells in the interstitium of the cortex and outer medulla .
	manualset3
231713	2	421635	7	NULL	NULL	0	NULL	Epo-TAg	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In transgenic mice bearing Epo-TAg at homologous and heterologous insertion sites , renal expression was restricted to a population of cells in the interstitium of the cortex and outer medulla .
	manualset3
231714	3	421635	7	NULL	NULL	0	NULL	 homologous insertion sites	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In transgenic mice bearing Epo-TAg at homologous and heterologous insertion sites , renal expression was restricted to a population of cells in the interstitium of the cortex and outer medulla .
	manualset3
231715	4	421635	7	NULL	NULL	0	NULL	 heterologous insertion sites	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In transgenic mice bearing Epo-TAg at homologous and heterologous insertion sites , renal expression was restricted to a population of cells in the interstitium of the cortex and outer medulla .
	manualset3
231716	5	421635	7	NULL	NULL	NULL	NULL	 renal expression	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In transgenic mice bearing Epo-TAg at homologous and heterologous insertion sites , renal expression was restricted to a population of cells in the interstitium of the cortex and outer medulla .
	manualset3
231717	6	421635	7	NULL	NULL	0	NULL	 population 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In transgenic mice bearing Epo-TAg at homologous and heterologous insertion sites , renal expression was restricted to a population of cells in the interstitium of the cortex and outer medulla .
	manualset3
231718	7	421635	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In transgenic mice bearing Epo-TAg at homologous and heterologous insertion sites , renal expression was restricted to a population of cells in the interstitium of the cortex and outer medulla .
	manualset3
231719	8	421635	7	NULL	NULL	0	NULL	interstitium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In transgenic mice bearing Epo-TAg at homologous and heterologous insertion sites , renal expression was restricted to a population of cells in the interstitium of the cortex and outer medulla .
	manualset3
231720	9	421635	7	NULL	NULL	0	NULL	cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In transgenic mice bearing Epo-TAg at homologous and heterologous insertion sites , renal expression was restricted to a population of cells in the interstitium of the cortex and outer medulla .
	manualset3
231721	10	421635	7	NULL	NULL	0	NULL	outer medulla 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In transgenic mice bearing Epo-TAg at homologous and heterologous insertion sites , renal expression was restricted to a population of cells in the interstitium of the cortex and outer medulla .
	manualset3
231722	1	421636	7	NULL	NULL	0	NULL	Effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of erythromycin and phosphomycin on the ingestion and destruction capacity of the human polymorphonuclear leukocyte ) .
	manualset3
231723	2	421636	7	NULL	NULL	0	NULL	erythromycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of erythromycin and phosphomycin on the ingestion and destruction capacity of the human polymorphonuclear leukocyte ) .
	manualset3
231724	3	421636	7	NULL	NULL	0	NULL	phosphomycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of erythromycin and phosphomycin on the ingestion and destruction capacity of the human polymorphonuclear leukocyte ) .
	manualset3
231726	4	421636	7	NULL	NULL	0	NULL	ingestion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of erythromycin and phosphomycin on the ingestion and destruction capacity of the human polymorphonuclear leukocyte ) .
	manualset3
231727	5	421636	7	NULL	NULL	0	NULL	destruction capacity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of erythromycin and phosphomycin on the ingestion and destruction capacity of the human polymorphonuclear leukocyte ) .
	manualset3
231728	6	421636	7	NULL	NULL	0	NULL	human polymorphonuclear leukocyte 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of erythromycin and phosphomycin on the ingestion and destruction capacity of the human polymorphonuclear leukocyte ) .
	manualset3
231729	1	421637	7	NULL	NULL	0	NULL	effects 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We evaluated effects of Wtip on podocyte cell-cell and cell-matrix contact organization using gain-of - and loss-of-function methods .
	manualset3
231730	2	421637	7	NULL	NULL	0	NULL	Wtip	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We evaluated effects of Wtip on podocyte cell-cell and cell-matrix contact organization using gain-of - and loss-of-function methods .
	manualset3
231731	3	421637	7	NULL	NULL	0	NULL	podocyte	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We evaluated effects of Wtip on podocyte cell-cell and cell-matrix contact organization using gain-of - and loss-of-function methods .
	manualset3
231732	4	421637	7	NULL	NULL	NULL	NULL	cell-cell contact organization	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We evaluated effects of Wtip on podocyte cell-cell and cell-matrix contact organization using gain-of - and loss-of-function methods .
	manualset3
231733	5	421637	7	NULL	NULL	0	NULL	gain-of -function methods	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We evaluated effects of Wtip on podocyte cell-cell and cell-matrix contact organization using gain-of - and loss-of-function methods .
	manualset3
231734	6	421637	7	NULL	NULL	0	NULL	loss-of-function methods 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We evaluated effects of Wtip on podocyte cell-cell and cell-matrix contact organization using gain-of - and loss-of-function methods .
	manualset3
235747	7	421637	7	NULL	NULL	NULL	NULL	cell-matrix contact organization	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We evaluated effects of Wtip on podocyte cell-cell and cell-matrix contact organization using gain-of - and loss-of-function methods .
	manualset3
231735	1	421638	7	NULL	NULL	0	NULL	Heat shock proteins 70 ( Hsp70 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat shock proteins 70 ( Hsp70 ) represent a ubiquitous and conserved family of molecular chaperones involved in a plethora of cellular processes .
	manualset3
231736	2	421638	7	NULL	NULL	0	NULL	conserved family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat shock proteins 70 ( Hsp70 ) represent a ubiquitous and conserved family of molecular chaperones involved in a plethora of cellular processes .
	manualset3
231737	3	421638	7	NULL	NULL	0	NULL	molecular chaperones	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat shock proteins 70 ( Hsp70 ) represent a ubiquitous and conserved family of molecular chaperones involved in a plethora of cellular processes .
	manualset3
231738	4	421638	7	NULL	NULL	0	NULL	cellular processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat shock proteins 70 ( Hsp70 ) represent a ubiquitous and conserved family of molecular chaperones involved in a plethora of cellular processes .
	manualset3
240135	5	421638	7	NULL	NULL	0	NULL	plethora 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Heat shock proteins 70 ( Hsp70 ) represent a ubiquitous and conserved family of molecular chaperones involved in a plethora of cellular processes .
	manualset3
231739	1	421639	7	NULL	NULL	NULL	NULL	intramuscular MU spikes 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The simultaneously recorded intramuscular MU spikes and surface electromyogram ( EMG ) data indicated that mean MU spike amplitude , firing frequency and the parameters of surface EMG power spectra ( mean power frequency and root mean square amplitude ) remained constant during the experiment with unhindered circulation , providing no electrophysiological signs of muscle fatigue .
	manualset3
231740	2	421639	7	NULL	NULL	0	NULL	mean MU spike amplitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The simultaneously recorded intramuscular MU spikes and surface electromyogram ( EMG ) data indicated that mean MU spike amplitude , firing frequency and the parameters of surface EMG power spectra ( mean power frequency and root mean square amplitude ) remained constant during the experiment with unhindered circulation , providing no electrophysiological signs of muscle fatigue .
	manualset3
231741	3	421639	7	NULL	NULL	0	NULL	 firing frequency 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The simultaneously recorded intramuscular MU spikes and surface electromyogram ( EMG ) data indicated that mean MU spike amplitude , firing frequency and the parameters of surface EMG power spectra ( mean power frequency and root mean square amplitude ) remained constant during the experiment with unhindered circulation , providing no electrophysiological signs of muscle fatigue .
	manualset3
231742	4	421639	7	NULL	NULL	0	NULL	parameters	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The simultaneously recorded intramuscular MU spikes and surface electromyogram ( EMG ) data indicated that mean MU spike amplitude , firing frequency and the parameters of surface EMG power spectra ( mean power frequency and root mean square amplitude ) remained constant during the experiment with unhindered circulation , providing no electrophysiological signs of muscle fatigue .
	manualset3
231743	5	421639	7	NULL	NULL	0	NULL	surface EMG power spectra	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The simultaneously recorded intramuscular MU spikes and surface electromyogram ( EMG ) data indicated that mean MU spike amplitude , firing frequency and the parameters of surface EMG power spectra ( mean power frequency and root mean square amplitude ) remained constant during the experiment with unhindered circulation , providing no electrophysiological signs of muscle fatigue .
	manualset3
231744	6	421639	7	NULL	NULL	0	NULL	mean power frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The simultaneously recorded intramuscular MU spikes and surface electromyogram ( EMG ) data indicated that mean MU spike amplitude , firing frequency and the parameters of surface EMG power spectra ( mean power frequency and root mean square amplitude ) remained constant during the experiment with unhindered circulation , providing no electrophysiological signs of muscle fatigue .
	manualset3
231745	7	421639	7	NULL	NULL	0	NULL	root mean square amplitude 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The simultaneously recorded intramuscular MU spikes and surface electromyogram ( EMG ) data indicated that mean MU spike amplitude , firing frequency and the parameters of surface EMG power spectra ( mean power frequency and root mean square amplitude ) remained constant during the experiment with unhindered circulation , providing no electrophysiological signs of muscle fatigue .
	manualset3
231746	8	421639	7	NULL	NULL	0	NULL	 experiment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The simultaneously recorded intramuscular MU spikes and surface electromyogram ( EMG ) data indicated that mean MU spike amplitude , firing frequency and the parameters of surface EMG power spectra ( mean power frequency and root mean square amplitude ) remained constant during the experiment with unhindered circulation , providing no electrophysiological signs of muscle fatigue .
	manualset3
231747	9	421639	7	NULL	NULL	0	NULL	unhindered circulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The simultaneously recorded intramuscular MU spikes and surface electromyogram ( EMG ) data indicated that mean MU spike amplitude , firing frequency and the parameters of surface EMG power spectra ( mean power frequency and root mean square amplitude ) remained constant during the experiment with unhindered circulation , providing no electrophysiological signs of muscle fatigue .
	manualset3
231748	10	421639	7	NULL	NULL	0	NULL	no electrophysiological signs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The simultaneously recorded intramuscular MU spikes and surface electromyogram ( EMG ) data indicated that mean MU spike amplitude , firing frequency and the parameters of surface EMG power spectra ( mean power frequency and root mean square amplitude ) remained constant during the experiment with unhindered circulation , providing no electrophysiological signs of muscle fatigue .
	manualset3
231749	11	421639	7	NULL	NULL	0	NULL	muscle fatigue 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The simultaneously recorded intramuscular MU spikes and surface electromyogram ( EMG ) data indicated that mean MU spike amplitude , firing frequency and the parameters of surface EMG power spectra ( mean power frequency and root mean square amplitude ) remained constant during the experiment with unhindered circulation , providing no electrophysiological signs of muscle fatigue .
	manualset3
235748	12	421639	7	NULL	NULL	NULL	NULL	surface electromyogram ( EMG ) data	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The simultaneously recorded intramuscular MU spikes and surface electromyogram ( EMG ) data indicated that mean MU spike amplitude , firing frequency and the parameters of surface EMG power spectra ( mean power frequency and root mean square amplitude ) remained constant during the experiment with unhindered circulation , providing no electrophysiological signs of muscle fatigue .
	manualset3
231750	1	421640	7	NULL	NULL	0	NULL	Promotion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Promotion of rational return of subject consciousness of enterprise social responsibility ) .
	manualset3
231751	2	421640	7	NULL	NULL	0	NULL	 rational return 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Promotion of rational return of subject consciousness of enterprise social responsibility ) .
	manualset3
231752	3	421640	7	NULL	NULL	0	NULL	subject consciousness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Promotion of rational return of subject consciousness of enterprise social responsibility ) .
	manualset3
231753	4	421640	7	NULL	NULL	0	NULL	enterprise social responsibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Promotion of rational return of subject consciousness of enterprise social responsibility ) .
	manualset3
231755	1	421641	7	NULL	NULL	0	NULL	two hypotheses	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we tested two hypotheses that pertain to population limitation : 1 .
	manualset3
231756	2	421641	7	NULL	NULL	0	NULL	population limitation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we tested two hypotheses that pertain to population limitation : 1 .
	manualset3
231757	3	421641	7	NULL	NULL	0	NULL	1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we tested two hypotheses that pertain to population limitation : 1 .
	manualset3
231771	1	421642	7	NULL	NULL	0	NULL	overexpression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The overexpression of STAT3 in melanoma cells is often observed and is suggested to be involved in tumorigenesis and development .
	manualset3
231772	2	421642	7	NULL	NULL	0	NULL	STAT3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The overexpression of STAT3 in melanoma cells is often observed and is suggested to be involved in tumorigenesis and development .
	manualset3
231773	3	421642	7	NULL	NULL	0	NULL	melanoma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The overexpression of STAT3 in melanoma cells is often observed and is suggested to be involved in tumorigenesis and development .
	manualset3
231774	4	421642	7	NULL	NULL	0	NULL	 tumorigenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The overexpression of STAT3 in melanoma cells is often observed and is suggested to be involved in tumorigenesis and development .
	manualset3
231777	5	421642	7	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The overexpression of STAT3 in melanoma cells is often observed and is suggested to be involved in tumorigenesis and development .
	manualset3
231778	1	421643	7	NULL	NULL	0	NULL	 analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An analysis of methodological fallacies indicates that observed effects and effect sizes can be underestimated , and that interventions may well have greater impact than this review was able to establish .
	manualset3
231780	2	421643	7	NULL	NULL	0	NULL	 methodological fallacies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An analysis of methodological fallacies indicates that observed effects and effect sizes can be underestimated , and that interventions may well have greater impact than this review was able to establish .
	manualset3
231781	3	421643	7	NULL	NULL	0	NULL	observed effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An analysis of methodological fallacies indicates that observed effects and effect sizes can be underestimated , and that interventions may well have greater impact than this review was able to establish .
	manualset3
231782	4	421643	7	NULL	NULL	0	NULL	effect sizes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An analysis of methodological fallacies indicates that observed effects and effect sizes can be underestimated , and that interventions may well have greater impact than this review was able to establish .
	manualset3
231783	5	421643	7	NULL	NULL	0	NULL	interventions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An analysis of methodological fallacies indicates that observed effects and effect sizes can be underestimated , and that interventions may well have greater impact than this review was able to establish .
	manualset3
231784	6	421643	7	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	An analysis of methodological fallacies indicates that observed effects and effect sizes can be underestimated , and that interventions may well have greater impact than this review was able to establish .
	manualset3
235749	7	421643	7	NULL	NULL	0	NULL	greater impact	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An analysis of methodological fallacies indicates that observed effects and effect sizes can be underestimated , and that interventions may well have greater impact than this review was able to establish .
	manualset3
231785	1	421644	7	NULL	NULL	0	NULL	Knowledge	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Knowledge of species specific pharmacology can be advantageous for drug discovery , where rats are frequently used as a model system .
	manualset3
231786	2	421644	7	NULL	NULL	0	NULL	species specific pharmacology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Knowledge of species specific pharmacology can be advantageous for drug discovery , where rats are frequently used as a model system .
	manualset3
231787	3	421644	7	NULL	NULL	0	NULL	drug discovery	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Knowledge of species specific pharmacology can be advantageous for drug discovery , where rats are frequently used as a model system .
	manualset3
231788	4	421644	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Knowledge of species specific pharmacology can be advantageous for drug discovery , where rats are frequently used as a model system .
	manualset3
231789	5	421644	7	NULL	NULL	0	NULL	model system	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Knowledge of species specific pharmacology can be advantageous for drug discovery , where rats are frequently used as a model system .
	manualset3
231790	1	421645	7	NULL	NULL	0	NULL	 tree	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The tree obtained indicated that there are two major clusters of vertebrate ERs : ERalpha and ERbeta .
	manualset3
231791	2	421645	7	NULL	NULL	0	NULL	two major clusters 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The tree obtained indicated that there are two major clusters of vertebrate ERs : ERalpha and ERbeta .
	manualset3
231792	3	421645	7	NULL	NULL	0	NULL	vertebrate ERs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The tree obtained indicated that there are two major clusters of vertebrate ERs : ERalpha and ERbeta .
	manualset3
231793	4	421645	7	NULL	NULL	0	NULL	ERalpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The tree obtained indicated that there are two major clusters of vertebrate ERs : ERalpha and ERbeta .
	manualset3
231794	5	421645	7	NULL	NULL	0	NULL	ERbeta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The tree obtained indicated that there are two major clusters of vertebrate ERs : ERalpha and ERbeta .
	manualset3
231795	1	421646	7	NULL	NULL	0	NULL	Role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of muscle microvasculature during hyperdynamic and hypodynamic phases of endotoxin shock in decerebrate rats .
	manualset3
231796	2	421646	7	NULL	NULL	0	NULL	muscle microvasculature	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of muscle microvasculature during hyperdynamic and hypodynamic phases of endotoxin shock in decerebrate rats .
	manualset3
231797	3	421646	7	NULL	NULL	0	NULL	hyperdynamic phases	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of muscle microvasculature during hyperdynamic and hypodynamic phases of endotoxin shock in decerebrate rats .
	manualset3
231798	4	421646	7	NULL	NULL	0	NULL	hypodynamic phases	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of muscle microvasculature during hyperdynamic and hypodynamic phases of endotoxin shock in decerebrate rats .
	manualset3
231799	5	421646	7	NULL	NULL	0	NULL	endotoxin shock	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of muscle microvasculature during hyperdynamic and hypodynamic phases of endotoxin shock in decerebrate rats .
	manualset3
231800	6	421646	7	NULL	NULL	0	NULL	decerebrate rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Role of muscle microvasculature during hyperdynamic and hypodynamic phases of endotoxin shock in decerebrate rats .
	manualset3
231801	1	421647	7	NULL	NULL	0	NULL	amino terminus	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino terminus of ADP-ribosylation factor ( ARF ) is a critical determinant of ARF activities and is a potent and specific inhibitor of protein transport .
	manualset3
231802	2	421647	7	NULL	NULL	0	NULL	 ADP-ribosylation factor ( ARF )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino terminus of ADP-ribosylation factor ( ARF ) is a critical determinant of ARF activities and is a potent and specific inhibitor of protein transport .
	manualset3
231803	3	421647	7	NULL	NULL	0	NULL	critical determinant 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino terminus of ADP-ribosylation factor ( ARF ) is a critical determinant of ARF activities and is a potent and specific inhibitor of protein transport .
	manualset3
231804	4	421647	7	NULL	NULL	0	NULL	ARF activities 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino terminus of ADP-ribosylation factor ( ARF ) is a critical determinant of ARF activities and is a potent and specific inhibitor of protein transport .
	manualset3
231805	5	421647	7	NULL	NULL	0	NULL	specific inhibitor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino terminus of ADP-ribosylation factor ( ARF ) is a critical determinant of ARF activities and is a potent and specific inhibitor of protein transport .
	manualset3
231806	6	421647	7	NULL	NULL	0	NULL	protein transport	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The amino terminus of ADP-ribosylation factor ( ARF ) is a critical determinant of ARF activities and is a potent and specific inhibitor of protein transport .
	manualset3
231807	1	421648	7	NULL	NULL	0	NULL	Significance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Significance of the hemodynamic theory of thrombogenesis and the results of its conservative-mechanic prevention and therapy ) .
	manualset3
231808	2	421648	7	NULL	NULL	0	NULL	hemodynamic theory	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Significance of the hemodynamic theory of thrombogenesis and the results of its conservative-mechanic prevention and therapy ) .
	manualset3
231809	3	421648	7	NULL	NULL	0	NULL	thrombogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Significance of the hemodynamic theory of thrombogenesis and the results of its conservative-mechanic prevention and therapy ) .
	manualset3
231810	4	421648	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Significance of the hemodynamic theory of thrombogenesis and the results of its conservative-mechanic prevention and therapy ) .
	manualset3
231811	5	421648	7	NULL	NULL	0	NULL	conservative-mechanic prevention	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Significance of the hemodynamic theory of thrombogenesis and the results of its conservative-mechanic prevention and therapy ) .
	manualset3
231812	6	421648	7	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Significance of the hemodynamic theory of thrombogenesis and the results of its conservative-mechanic prevention and therapy ) .
	manualset3
231813	1	421649	7	NULL	NULL	0	NULL	analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An analysis of our experimental data based on a ` single-shell ' model showed that conductivity and permittivity of the membrane of pre - and post-fusion myoblasts varied significantly and abruptly .
	manualset3
231814	2	421649	7	NULL	NULL	NULL	NULL	experimental data	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An analysis of our experimental data based on a ` single-shell ' model showed that conductivity and permittivity of the membrane of pre - and post-fusion myoblasts varied significantly and abruptly .
	manualset3
231815	3	421649	7	NULL	NULL	0	NULL	` single-shell ' model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	An analysis of our experimental data based on a ` single-shell ' model showed that conductivity and permittivity of the membrane of pre - and post-fusion myoblasts varied significantly and abruptly .
	manualset3
231816	4	421649	7	NULL	NULL	0	NULL	conductivity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An analysis of our experimental data based on a ` single-shell ' model showed that conductivity and permittivity of the membrane of pre - and post-fusion myoblasts varied significantly and abruptly .
	manualset3
231817	5	421649	7	NULL	NULL	0	NULL	permittivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An analysis of our experimental data based on a ` single-shell ' model showed that conductivity and permittivity of the membrane of pre - and post-fusion myoblasts varied significantly and abruptly .
	manualset3
231818	6	421649	7	NULL	NULL	NULL	NULL	pre -fusion myoblasts	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An analysis of our experimental data based on a ` single-shell ' model showed that conductivity and permittivity of the membrane of pre - and post-fusion myoblasts varied significantly and abruptly .
	manualset3
231819	7	421649	7	NULL	NULL	NULL	NULL	post-fusion myoblasts	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An analysis of our experimental data based on a ` single-shell ' model showed that conductivity and permittivity of the membrane of pre - and post-fusion myoblasts varied significantly and abruptly .
	manualset3
235750	8	421649	7	NULL	NULL	0	NULL	membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	An analysis of our experimental data based on a ` single-shell ' model showed that conductivity and permittivity of the membrane of pre - and post-fusion myoblasts varied significantly and abruptly .
	manualset3
231820	1	421650	7	NULL	NULL	0	NULL	intracellular biochemical changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The intracellular biochemical changes that occur leading to Cld-induced nephrotoxicity may involve lipid peroxidation and/or mitochondrial injury .
	manualset3
231821	2	421650	7	NULL	NULL	0	NULL	Cld-induced nephrotoxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The intracellular biochemical changes that occur leading to Cld-induced nephrotoxicity may involve lipid peroxidation and/or mitochondrial injury .
	manualset3
231822	3	421650	7	NULL	NULL	0	NULL	lipid peroxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The intracellular biochemical changes that occur leading to Cld-induced nephrotoxicity may involve lipid peroxidation and/or mitochondrial injury .
	manualset3
231823	4	421650	7	NULL	NULL	0	NULL	mitochondrial injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The intracellular biochemical changes that occur leading to Cld-induced nephrotoxicity may involve lipid peroxidation and/or mitochondrial injury .
	manualset3
231824	1	421651	7	NULL	NULL	0	NULL	vestigial plastid	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	They contain a vestigial plastid , the apicoplast , that originated through the secondary endosymbiosis of the photosynthetic unicellular alga .
	manualset3
231825	2	421651	7	NULL	NULL	0	NULL	apicoplast	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	They contain a vestigial plastid , the apicoplast , that originated through the secondary endosymbiosis of the photosynthetic unicellular alga .
	manualset3
231826	3	421651	7	NULL	NULL	0	NULL	 secondary endosymbiosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	They contain a vestigial plastid , the apicoplast , that originated through the secondary endosymbiosis of the photosynthetic unicellular alga .
	manualset3
231827	4	421651	7	NULL	NULL	0	NULL	photosynthetic unicellular alga	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	They contain a vestigial plastid , the apicoplast , that originated through the secondary endosymbiosis of the photosynthetic unicellular alga .
	manualset3
231828	1	421652	7	NULL	NULL	0	NULL	assignments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These assignments were the basis to investigate the interaction sites between the protein folding helper enzyme SlyD ( 1-165 ) ( SlyD * ) from Escherichia coli ( E. coli ) and this kinetic intermediate at a residue resolution .
	manualset3
231829	2	421652	7	NULL	NULL	0	NULL	interaction sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These assignments were the basis to investigate the interaction sites between the protein folding helper enzyme SlyD ( 1-165 ) ( SlyD * ) from Escherichia coli ( E. coli ) and this kinetic intermediate at a residue resolution .
	manualset3
231830	3	421652	7	NULL	NULL	0	NULL	protein folding helper enzyme SlyD	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These assignments were the basis to investigate the interaction sites between the protein folding helper enzyme SlyD ( 1-165 ) ( SlyD * ) from Escherichia coli ( E. coli ) and this kinetic intermediate at a residue resolution .
	manualset3
231831	4	421652	7	NULL	NULL	0	NULL	1-165	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These assignments were the basis to investigate the interaction sites between the protein folding helper enzyme SlyD ( 1-165 ) ( SlyD * ) from Escherichia coli ( E. coli ) and this kinetic intermediate at a residue resolution .
	manualset3
231832	5	421652	7	NULL	NULL	0	NULL	SlyD *	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These assignments were the basis to investigate the interaction sites between the protein folding helper enzyme SlyD ( 1-165 ) ( SlyD * ) from Escherichia coli ( E. coli ) and this kinetic intermediate at a residue resolution .
	manualset3
231833	6	421652	7	NULL	NULL	0	NULL	Escherichia coli ( E. coli )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These assignments were the basis to investigate the interaction sites between the protein folding helper enzyme SlyD ( 1-165 ) ( SlyD * ) from Escherichia coli ( E. coli ) and this kinetic intermediate at a residue resolution .
	manualset3
231834	7	421652	7	NULL	NULL	0	NULL	kinetic intermediate	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	These assignments were the basis to investigate the interaction sites between the protein folding helper enzyme SlyD ( 1-165 ) ( SlyD * ) from Escherichia coli ( E. coli ) and this kinetic intermediate at a residue resolution .
	manualset3
231835	8	421652	7	NULL	NULL	0	NULL	residue resolution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These assignments were the basis to investigate the interaction sites between the protein folding helper enzyme SlyD ( 1-165 ) ( SlyD * ) from Escherichia coli ( E. coli ) and this kinetic intermediate at a residue resolution .
	manualset3
231836	1	421653	7	NULL	NULL	0	NULL	Treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of chronic hepatitis C with consensus interferon : a multicenter , randomized , controlled trial .
	manualset3
231837	2	421653	7	NULL	NULL	0	NULL	chronic hepatitis C 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of chronic hepatitis C with consensus interferon : a multicenter , randomized , controlled trial .
	manualset3
231838	3	421653	7	NULL	NULL	0	NULL	consensus interferon	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of chronic hepatitis C with consensus interferon : a multicenter , randomized , controlled trial .
	manualset3
231839	4	421653	7	NULL	NULL	0	NULL	multicenter , randomized , controlled trial	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment of chronic hepatitis C with consensus interferon : a multicenter , randomized , controlled trial .
	manualset3
231840	1	421654	7	NULL	NULL	0	NULL	Synthesis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Synthesis and antitrichinellosis activity of some 2-substituted - ( 1 , 3 ) thiazolo ( 3 , 2-a ) benzimidazol-3 ( 2H ) - ones .
	manualset3
231841	2	421654	7	NULL	NULL	0	NULL	antitrichinellosis activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Synthesis and antitrichinellosis activity of some 2-substituted - ( 1 , 3 ) thiazolo ( 3 , 2-a ) benzimidazol-3 ( 2H ) - ones .
	manualset3
231842	3	421654	7	NULL	NULL	0	NULL	2-substituted - ( 1 , 3 ) thiazolo ( 3 , 2-a ) benzimidazol-3 ( 2H ) - ones	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Synthesis and antitrichinellosis activity of some 2-substituted - ( 1 , 3 ) thiazolo ( 3 , 2-a ) benzimidazol-3 ( 2H ) - ones .
	manualset3
231843	1	421655	7	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we evaluated the effect of the activation of an artificial death switch ( iCaspase-9 ) expressed in neovascular endothelial cells on the progression of oral tumors .
	manualset3
231844	2	421655	7	NULL	NULL	0	NULL	 activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we evaluated the effect of the activation of an artificial death switch ( iCaspase-9 ) expressed in neovascular endothelial cells on the progression of oral tumors .
	manualset3
231845	3	421655	7	NULL	NULL	0	NULL	artificial death switch 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we evaluated the effect of the activation of an artificial death switch ( iCaspase-9 ) expressed in neovascular endothelial cells on the progression of oral tumors .
	manualset3
231846	4	421655	7	NULL	NULL	0	NULL	 iCaspase-9	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we evaluated the effect of the activation of an artificial death switch ( iCaspase-9 ) expressed in neovascular endothelial cells on the progression of oral tumors .
	manualset3
231847	5	421655	7	NULL	NULL	0	NULL	neovascular endothelial cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we evaluated the effect of the activation of an artificial death switch ( iCaspase-9 ) expressed in neovascular endothelial cells on the progression of oral tumors .
	manualset3
231848	6	421655	7	NULL	NULL	0	NULL	progression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we evaluated the effect of the activation of an artificial death switch ( iCaspase-9 ) expressed in neovascular endothelial cells on the progression of oral tumors .
	manualset3
231849	7	421655	7	NULL	NULL	0	NULL	oral tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Here , we evaluated the effect of the activation of an artificial death switch ( iCaspase-9 ) expressed in neovascular endothelial cells on the progression of oral tumors .
	manualset3
231850	1	421656	7	NULL	NULL	0	NULL	animal model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	An animal model of AD-like pruritus would contribute to a better understanding of AD and could lead to the development of safe and effective antipruritic agents .
	manualset3
231851	2	421656	7	NULL	NULL	0	NULL	AD-like pruritus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	An animal model of AD-like pruritus would contribute to a better understanding of AD and could lead to the development of safe and effective antipruritic agents .
	manualset3
231852	3	421656	7	NULL	NULL	0	NULL	understanding 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An animal model of AD-like pruritus would contribute to a better understanding of AD and could lead to the development of safe and effective antipruritic agents .
	manualset3
231853	4	421656	7	NULL	NULL	0	NULL	 AD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	An animal model of AD-like pruritus would contribute to a better understanding of AD and could lead to the development of safe and effective antipruritic agents .
	manualset3
231854	5	421656	7	NULL	NULL	0	NULL	 development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An animal model of AD-like pruritus would contribute to a better understanding of AD and could lead to the development of safe and effective antipruritic agents .
	manualset3
231855	6	421656	7	NULL	NULL	0	NULL	antipruritic agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An animal model of AD-like pruritus would contribute to a better understanding of AD and could lead to the development of safe and effective antipruritic agents .
	manualset3
231856	1	421657	7	NULL	NULL	0	NULL	Nursing care	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nursing care of patients with ocular manifestations of human immunodeficiency virus infection .
	manualset3
231857	2	421657	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nursing care of patients with ocular manifestations of human immunodeficiency virus infection .
	manualset3
231858	3	421657	7	NULL	NULL	0	NULL	ocular manifestations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Nursing care of patients with ocular manifestations of human immunodeficiency virus infection .
	manualset3
231859	4	421657	7	NULL	NULL	0	NULL	human immunodeficiency virus infection	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Nursing care of patients with ocular manifestations of human immunodeficiency virus infection .
	manualset3
231860	1	421658	7	NULL	NULL	NULL	NULL	Treatment 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Treatment with intravenous chlormethiazole resulted in rapid control of her myoclonic attacks , followed by slower but complete resolution of the opsoclonus .
	manualset3
231861	2	421658	7	NULL	NULL	0	NULL	intravenous chlormethiazole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with intravenous chlormethiazole resulted in rapid control of her myoclonic attacks , followed by slower but complete resolution of the opsoclonus .
	manualset3
231862	3	421658	7	NULL	NULL	0	NULL	rapid control 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with intravenous chlormethiazole resulted in rapid control of her myoclonic attacks , followed by slower but complete resolution of the opsoclonus .
	manualset3
231863	4	421658	7	NULL	NULL	0	NULL	 myoclonic attacks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with intravenous chlormethiazole resulted in rapid control of her myoclonic attacks , followed by slower but complete resolution of the opsoclonus .
	manualset3
231864	5	421658	7	NULL	NULL	0	NULL	complete resolution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with intravenous chlormethiazole resulted in rapid control of her myoclonic attacks , followed by slower but complete resolution of the opsoclonus .
	manualset3
231865	6	421658	7	NULL	NULL	0	NULL	opsoclonus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Treatment with intravenous chlormethiazole resulted in rapid control of her myoclonic attacks , followed by slower but complete resolution of the opsoclonus .
	manualset3
231866	1	421659	7	NULL	NULL	0	NULL	Intracellular recordings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular recordings were made from isolated frog sciatic-sartorius nerve-muscle preparations , and the effects of sphingosine 1-phosphate ( S1-P ) on miniature endplate potentials ( MEPPs ) were studied .
	manualset3
231867	2	421659	7	NULL	NULL	0	NULL	 isolated frog sciatic-sartorius nerve-muscle preparations	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular recordings were made from isolated frog sciatic-sartorius nerve-muscle preparations , and the effects of sphingosine 1-phosphate ( S1-P ) on miniature endplate potentials ( MEPPs ) were studied .
	manualset3
231868	3	421659	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular recordings were made from isolated frog sciatic-sartorius nerve-muscle preparations , and the effects of sphingosine 1-phosphate ( S1-P ) on miniature endplate potentials ( MEPPs ) were studied .
	manualset3
231869	4	421659	7	NULL	NULL	NULL	NULL	sphingosine 1-phosphate ( S1-P )	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Intracellular recordings were made from isolated frog sciatic-sartorius nerve-muscle preparations , and the effects of sphingosine 1-phosphate ( S1-P ) on miniature endplate potentials ( MEPPs ) were studied .
	manualset3
231870	5	421659	7	NULL	NULL	NULL	NULL	miniature endplate potentials ( MEPPs )	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Intracellular recordings were made from isolated frog sciatic-sartorius nerve-muscle preparations , and the effects of sphingosine 1-phosphate ( S1-P ) on miniature endplate potentials ( MEPPs ) were studied .
	manualset3
231871	1	421660	7	NULL	NULL	0	NULL	ABA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that ABA is without significant Ca2 + modulatory activity in this smooth muscle preparation but the ABA analog SD217595 possesses strong Ca2 + entry blocking ability .
	manualset3
231872	2	421660	7	NULL	NULL	0	NULL	Ca2 + modulatory activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that ABA is without significant Ca2 + modulatory activity in this smooth muscle preparation but the ABA analog SD217595 possesses strong Ca2 + entry blocking ability .
	manualset3
231873	3	421660	7	NULL	NULL	0	NULL	smooth muscle preparation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that ABA is without significant Ca2 + modulatory activity in this smooth muscle preparation but the ABA analog SD217595 possesses strong Ca2 + entry blocking ability .
	manualset3
231874	4	421660	7	NULL	NULL	0	NULL	ABA analog SD217595	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that ABA is without significant Ca2 + modulatory activity in this smooth muscle preparation but the ABA analog SD217595 possesses strong Ca2 + entry blocking ability .
	manualset3
231875	5	421660	7	NULL	NULL	0	NULL	strong Ca2 + entry blocking ability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that ABA is without significant Ca2 + modulatory activity in this smooth muscle preparation but the ABA analog SD217595 possesses strong Ca2 + entry blocking ability .
	manualset3
231876	1	421661	7	NULL	NULL	0	NULL	Angiotensin-converting enzyme ( ACE ) inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin-converting enzyme ( ACE ) inhibitors and angiotensin receptor blockers ( ARB ) have beneficial effects on proteinuria and declining renal function that appear to be mediated by factors additional to their effects on BP .
	manualset3
231877	2	421661	7	NULL	NULL	0	NULL	angiotensin receptor blockers ( ARB )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin-converting enzyme ( ACE ) inhibitors and angiotensin receptor blockers ( ARB ) have beneficial effects on proteinuria and declining renal function that appear to be mediated by factors additional to their effects on BP .
	manualset3
231878	3	421661	7	NULL	NULL	0	NULL	beneficial effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin-converting enzyme ( ACE ) inhibitors and angiotensin receptor blockers ( ARB ) have beneficial effects on proteinuria and declining renal function that appear to be mediated by factors additional to their effects on BP .
	manualset3
231879	4	421661	7	NULL	NULL	0	NULL	proteinuria 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin-converting enzyme ( ACE ) inhibitors and angiotensin receptor blockers ( ARB ) have beneficial effects on proteinuria and declining renal function that appear to be mediated by factors additional to their effects on BP .
	manualset3
231880	5	421661	7	NULL	NULL	0	NULL	renal function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin-converting enzyme ( ACE ) inhibitors and angiotensin receptor blockers ( ARB ) have beneficial effects on proteinuria and declining renal function that appear to be mediated by factors additional to their effects on BP .
	manualset3
231881	6	421661	7	NULL	NULL	0	NULL	factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin-converting enzyme ( ACE ) inhibitors and angiotensin receptor blockers ( ARB ) have beneficial effects on proteinuria and declining renal function that appear to be mediated by factors additional to their effects on BP .
	manualset3
231882	7	421661	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin-converting enzyme ( ACE ) inhibitors and angiotensin receptor blockers ( ARB ) have beneficial effects on proteinuria and declining renal function that appear to be mediated by factors additional to their effects on BP .
	manualset3
231883	8	421661	7	NULL	NULL	0	NULL	BP	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin-converting enzyme ( ACE ) inhibitors and angiotensin receptor blockers ( ARB ) have beneficial effects on proteinuria and declining renal function that appear to be mediated by factors additional to their effects on BP .
	manualset3
231884	1	421662	7	NULL	NULL	0	NULL	anterolateral branch 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An anterolateral branch of the circumflex coronary artery was occluded for 30 minutes and reperfused for 2 hours .
	manualset3
231885	2	421662	7	NULL	NULL	0	NULL	circumflex coronary artery 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An anterolateral branch of the circumflex coronary artery was occluded for 30 minutes and reperfused for 2 hours .
	manualset3
231886	3	421662	7	NULL	NULL	0	NULL	30 minutes	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	An anterolateral branch of the circumflex coronary artery was occluded for 30 minutes and reperfused for 2 hours .
	manualset3
231887	4	421662	7	NULL	NULL	0	NULL	 2 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	An anterolateral branch of the circumflex coronary artery was occluded for 30 minutes and reperfused for 2 hours .
	manualset3
231888	1	421663	7	NULL	NULL	0	NULL	Analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of lectin properties with membrane ultrafiltration and high-pressure liquid chromatography .
	manualset3
231889	2	421663	7	NULL	NULL	0	NULL	 lectin properties	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of lectin properties with membrane ultrafiltration and high-pressure liquid chromatography .
	manualset3
231890	3	421663	7	NULL	NULL	0	NULL	membrane ultrafiltration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of lectin properties with membrane ultrafiltration and high-pressure liquid chromatography .
	manualset3
231891	4	421663	7	NULL	NULL	0	NULL	high-pressure liquid chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of lectin properties with membrane ultrafiltration and high-pressure liquid chromatography .
	manualset3
231892	1	421664	7	NULL	NULL	0	NULL	Ears reshaped with suture	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ears reshaped with suture alone maintained a folded angle close to the original right angle .
	manualset3
231893	2	421664	7	NULL	NULL	0	NULL	folded angle	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ears reshaped with suture alone maintained a folded angle close to the original right angle .
	manualset3
231894	3	421664	7	NULL	NULL	0	NULL	original right angle 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ears reshaped with suture alone maintained a folded angle close to the original right angle .
	manualset3
231895	1	421665	7	NULL	NULL	0	NULL	Predictions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictions averaged over time showed mean PIR between 36 % and 48 % , which is below the population immunity thresholds for eradication approximated from R0 estimates .
	manualset3
231896	2	421665	7	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictions averaged over time showed mean PIR between 36 % and 48 % , which is below the population immunity thresholds for eradication approximated from R0 estimates .
	manualset3
231897	3	421665	7	NULL	NULL	0	NULL	PIR 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictions averaged over time showed mean PIR between 36 % and 48 % , which is below the population immunity thresholds for eradication approximated from R0 estimates .
	manualset3
231898	4	421665	7	NULL	NULL	0	NULL	36 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictions averaged over time showed mean PIR between 36 % and 48 % , which is below the population immunity thresholds for eradication approximated from R0 estimates .
	manualset3
231899	5	421665	7	NULL	NULL	0	NULL	48 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictions averaged over time showed mean PIR between 36 % and 48 % , which is below the population immunity thresholds for eradication approximated from R0 estimates .
	manualset3
231900	6	421665	7	NULL	NULL	0	NULL	population immunity thresholds	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictions averaged over time showed mean PIR between 36 % and 48 % , which is below the population immunity thresholds for eradication approximated from R0 estimates .
	manualset3
231901	7	421665	7	NULL	NULL	0	NULL	eradication	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictions averaged over time showed mean PIR between 36 % and 48 % , which is below the population immunity thresholds for eradication approximated from R0 estimates .
	manualset3
231902	8	421665	7	NULL	NULL	0	NULL	R0 estimates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictions averaged over time showed mean PIR between 36 % and 48 % , which is below the population immunity thresholds for eradication approximated from R0 estimates .
	manualset3
231903	1	421666	7	NULL	NULL	0	NULL	anti-c-erbB-2 mAb ( ICR12 ) 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	An anti-c-erbB-2 mAb ( ICR12 ) showed similar effects on basal or ligand-modulated expression of VEGF in these cell lines , although to a lesser extent .
	manualset3
231904	2	421666	7	NULL	NULL	0	NULL	similar effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An anti-c-erbB-2 mAb ( ICR12 ) showed similar effects on basal or ligand-modulated expression of VEGF in these cell lines , although to a lesser extent .
	manualset3
231905	3	421666	7	NULL	NULL	0	NULL	basal-modulated expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An anti-c-erbB-2 mAb ( ICR12 ) showed similar effects on basal or ligand-modulated expression of VEGF in these cell lines , although to a lesser extent .
	manualset3
231906	4	421666	7	NULL	NULL	0	NULL	ligand-modulated expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An anti-c-erbB-2 mAb ( ICR12 ) showed similar effects on basal or ligand-modulated expression of VEGF in these cell lines , although to a lesser extent .
	manualset3
231907	5	421666	7	NULL	NULL	0	NULL	VEGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	An anti-c-erbB-2 mAb ( ICR12 ) showed similar effects on basal or ligand-modulated expression of VEGF in these cell lines , although to a lesser extent .
	manualset3
231908	6	421666	7	NULL	NULL	0	NULL	cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	An anti-c-erbB-2 mAb ( ICR12 ) showed similar effects on basal or ligand-modulated expression of VEGF in these cell lines , although to a lesser extent .
	manualset3
231909	1	421667	7	NULL	NULL	0	NULL	rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of hydrogen ion secretion increases linearly with pH over the intragastric range of pH 4.4 to 9.4 .
	manualset3
231910	2	421667	7	NULL	NULL	0	NULL	hydrogen ion secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of hydrogen ion secretion increases linearly with pH over the intragastric range of pH 4.4 to 9.4 .
	manualset3
231911	3	421667	7	NULL	NULL	0	NULL	pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of hydrogen ion secretion increases linearly with pH over the intragastric range of pH 4.4 to 9.4 .
	manualset3
231912	4	421667	7	NULL	NULL	0	NULL	intragastric range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of hydrogen ion secretion increases linearly with pH over the intragastric range of pH 4.4 to 9.4 .
	manualset3
231913	5	421667	7	NULL	NULL	0	NULL	 pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of hydrogen ion secretion increases linearly with pH over the intragastric range of pH 4.4 to 9.4 .
	manualset3
231914	6	421667	7	NULL	NULL	0	NULL	4.4	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of hydrogen ion secretion increases linearly with pH over the intragastric range of pH 4.4 to 9.4 .
	manualset3
231915	7	421667	7	NULL	NULL	0	NULL	9.4 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of hydrogen ion secretion increases linearly with pH over the intragastric range of pH 4.4 to 9.4 .
	manualset3
231916	1	421668	7	NULL	NULL	0	NULL	Complementary surgical treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Complementary surgical treatment was carried out on `` accessory '' arterial lesions in 33 cases ; 32 sympathectomies for distal lower limb lesions and I femoro-popliteal bypass after iliac PTA .
	manualset3
231917	2	421668	7	NULL	NULL	0	NULL	`` accessory '' arterial lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Complementary surgical treatment was carried out on `` accessory '' arterial lesions in 33 cases ; 32 sympathectomies for distal lower limb lesions and I femoro-popliteal bypass after iliac PTA .
	manualset3
231918	3	421668	7	NULL	NULL	0	NULL	33 cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Complementary surgical treatment was carried out on `` accessory '' arterial lesions in 33 cases ; 32 sympathectomies for distal lower limb lesions and I femoro-popliteal bypass after iliac PTA .
	manualset3
231919	4	421668	7	NULL	NULL	0	NULL	32 sympathectomies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Complementary surgical treatment was carried out on `` accessory '' arterial lesions in 33 cases ; 32 sympathectomies for distal lower limb lesions and I femoro-popliteal bypass after iliac PTA .
	manualset3
231920	5	421668	7	NULL	NULL	0	NULL	distal lower limb lesions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Complementary surgical treatment was carried out on `` accessory '' arterial lesions in 33 cases ; 32 sympathectomies for distal lower limb lesions and I femoro-popliteal bypass after iliac PTA .
	manualset3
231921	6	421668	7	NULL	NULL	0	NULL	I femoro-popliteal bypass	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Complementary surgical treatment was carried out on `` accessory '' arterial lesions in 33 cases ; 32 sympathectomies for distal lower limb lesions and I femoro-popliteal bypass after iliac PTA .
	manualset3
231922	7	421668	7	NULL	NULL	0	NULL	iliac PTA 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Complementary surgical treatment was carried out on `` accessory '' arterial lesions in 33 cases ; 32 sympathectomies for distal lower limb lesions and I femoro-popliteal bypass after iliac PTA .
	manualset3
231923	1	421669	7	NULL	NULL	0	NULL	 calcium ion	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	It appeared that calcium and sodium ions may not take part in the effects of d-amphetamine on the frequency of the portal vein .
	manualset3
231924	2	421669	7	NULL	NULL	0	NULL	sodium ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	It appeared that calcium and sodium ions may not take part in the effects of d-amphetamine on the frequency of the portal vein .
	manualset3
231925	3	421669	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It appeared that calcium and sodium ions may not take part in the effects of d-amphetamine on the frequency of the portal vein .
	manualset3
231926	4	421669	7	NULL	NULL	0	NULL	d-amphetamine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	It appeared that calcium and sodium ions may not take part in the effects of d-amphetamine on the frequency of the portal vein .
	manualset3
231927	5	421669	7	NULL	NULL	0	NULL	 frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It appeared that calcium and sodium ions may not take part in the effects of d-amphetamine on the frequency of the portal vein .
	manualset3
231928	6	421669	7	NULL	NULL	0	NULL	 portal vein	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It appeared that calcium and sodium ions may not take part in the effects of d-amphetamine on the frequency of the portal vein .
	manualset3
231929	1	421670	7	NULL	NULL	0	NULL	Infections 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Infections , especially with penicillin-resistant staphylococci , following thoracic surgery treated with large doses of penicillin .
	manualset3
231930	2	421670	7	NULL	NULL	0	NULL	penicillin-resistant staphylococci 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Infections , especially with penicillin-resistant staphylococci , following thoracic surgery treated with large doses of penicillin .
	manualset3
231931	3	421670	7	NULL	NULL	0	NULL	thoracic surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Infections , especially with penicillin-resistant staphylococci , following thoracic surgery treated with large doses of penicillin .
	manualset3
231932	4	421670	7	NULL	NULL	0	NULL	large doses 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Infections , especially with penicillin-resistant staphylococci , following thoracic surgery treated with large doses of penicillin .
	manualset3
231933	5	421670	7	NULL	NULL	0	NULL	penicillin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Infections , especially with penicillin-resistant staphylococci , following thoracic surgery treated with large doses of penicillin .
	manualset3
231934	1	421671	7	NULL	NULL	0	NULL	reproducibility	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For reproducibility , the coefficient of variation ( CV ) was 0.52-0 .70 % in vitro .
	manualset3
231935	2	421671	7	NULL	NULL	0	NULL	coefficient of variation ( CV )	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	For reproducibility , the coefficient of variation ( CV ) was 0.52-0 .70 % in vitro .
	manualset3
231936	3	421671	7	NULL	NULL	0	NULL	0.52-0 .70 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For reproducibility , the coefficient of variation ( CV ) was 0.52-0 .70 % in vitro .
	manualset3
231937	1	421672	7	NULL	NULL	0	NULL	tegmentum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Inside the tegmentum , specific intercellular cavities were found filled with a fibrillar network .
	manualset3
231938	2	421672	7	NULL	NULL	0	NULL	 intercellular cavities	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Inside the tegmentum , specific intercellular cavities were found filled with a fibrillar network .
	manualset3
231939	3	421672	7	NULL	NULL	0	NULL	 fibrillar network 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Inside the tegmentum , specific intercellular cavities were found filled with a fibrillar network .
	manualset3
231940	1	421673	7	NULL	NULL	0	NULL	horses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	All horses had degenerative lesions in peripheral and intramuscular nerves .
	manualset3
231941	2	421673	7	NULL	NULL	0	NULL	degenerative lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All horses had degenerative lesions in peripheral and intramuscular nerves .
	manualset3
231942	3	421673	7	NULL	NULL	0	NULL	peripheral nerves	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	All horses had degenerative lesions in peripheral and intramuscular nerves .
	manualset3
231943	4	421673	7	NULL	NULL	0	NULL	intramuscular nerves	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	All horses had degenerative lesions in peripheral and intramuscular nerves .
	manualset3
231944	1	421674	7	NULL	NULL	0	NULL	 antigen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	An antigen encoded by the latency-associated transcript in neuronal cell cultures latently infected with herpes simplex virus type 1 .
	manualset3
231945	2	421674	7	NULL	NULL	0	NULL	latency-associated transcript	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	An antigen encoded by the latency-associated transcript in neuronal cell cultures latently infected with herpes simplex virus type 1 .
	manualset3
231946	3	421674	7	NULL	NULL	0	NULL	neuronal cell cultures 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	An antigen encoded by the latency-associated transcript in neuronal cell cultures latently infected with herpes simplex virus type 1 .
	manualset3
231947	4	421674	7	NULL	NULL	0	NULL	herpes simplex virus type 1	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	An antigen encoded by the latency-associated transcript in neuronal cell cultures latently infected with herpes simplex virus type 1 .
	manualset3
231948	1	421675	7	NULL	NULL	0	NULL	 transcriptional profile	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We compare the transcriptional profile of A. halleri with that of its sister nonaccumulator species , Arabidopsis petraea , and between accumulator and nonaccumulator F ( 3 ) s derived from the cross between the two species .
	manualset3
231949	2	421675	7	NULL	NULL	0	NULL	A. halleri	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We compare the transcriptional profile of A. halleri with that of its sister nonaccumulator species , Arabidopsis petraea , and between accumulator and nonaccumulator F ( 3 ) s derived from the cross between the two species .
	manualset3
231950	3	421675	7	NULL	NULL	0	NULL	sister nonaccumulator species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We compare the transcriptional profile of A. halleri with that of its sister nonaccumulator species , Arabidopsis petraea , and between accumulator and nonaccumulator F ( 3 ) s derived from the cross between the two species .
	manualset3
231951	4	421675	7	NULL	NULL	0	NULL	Arabidopsis petraea	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We compare the transcriptional profile of A. halleri with that of its sister nonaccumulator species , Arabidopsis petraea , and between accumulator and nonaccumulator F ( 3 ) s derived from the cross between the two species .
	manualset3
231952	5	421675	7	NULL	NULL	0	NULL	accumulator F ( 3 ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We compare the transcriptional profile of A. halleri with that of its sister nonaccumulator species , Arabidopsis petraea , and between accumulator and nonaccumulator F ( 3 ) s derived from the cross between the two species .
	manualset3
231953	6	421675	7	NULL	NULL	0	NULL	nonaccumulator F ( 3 )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We compare the transcriptional profile of A. halleri with that of its sister nonaccumulator species , Arabidopsis petraea , and between accumulator and nonaccumulator F ( 3 ) s derived from the cross between the two species .
	manualset3
231954	7	421675	7	NULL	NULL	0	NULL	cross	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We compare the transcriptional profile of A. halleri with that of its sister nonaccumulator species , Arabidopsis petraea , and between accumulator and nonaccumulator F ( 3 ) s derived from the cross between the two species .
	manualset3
231955	8	421675	7	NULL	NULL	0	NULL	 two species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We compare the transcriptional profile of A. halleri with that of its sister nonaccumulator species , Arabidopsis petraea , and between accumulator and nonaccumulator F ( 3 ) s derived from the cross between the two species .
	manualset3
231956	1	421676	7	NULL	NULL	0	NULL	cascade of events	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the exact cascade of events that culminate into a migraine attack remains elusive , the mechanisms that underlie the manifestation of migraine pain have been better studied , and results obtained in animal models provide insight into the human situation .
	manualset3
231957	2	421676	7	NULL	NULL	0	NULL	migraine attack	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the exact cascade of events that culminate into a migraine attack remains elusive , the mechanisms that underlie the manifestation of migraine pain have been better studied , and results obtained in animal models provide insight into the human situation .
	manualset3
231958	3	421676	7	NULL	NULL	0	NULL	mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the exact cascade of events that culminate into a migraine attack remains elusive , the mechanisms that underlie the manifestation of migraine pain have been better studied , and results obtained in animal models provide insight into the human situation .
	manualset3
231959	4	421676	7	NULL	NULL	0	NULL	manifestation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the exact cascade of events that culminate into a migraine attack remains elusive , the mechanisms that underlie the manifestation of migraine pain have been better studied , and results obtained in animal models provide insight into the human situation .
	manualset3
231960	5	421676	7	NULL	NULL	0	NULL	migraine pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the exact cascade of events that culminate into a migraine attack remains elusive , the mechanisms that underlie the manifestation of migraine pain have been better studied , and results obtained in animal models provide insight into the human situation .
	manualset3
231961	6	421676	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the exact cascade of events that culminate into a migraine attack remains elusive , the mechanisms that underlie the manifestation of migraine pain have been better studied , and results obtained in animal models provide insight into the human situation .
	manualset3
231962	7	421676	7	NULL	NULL	0	NULL	animal models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the exact cascade of events that culminate into a migraine attack remains elusive , the mechanisms that underlie the manifestation of migraine pain have been better studied , and results obtained in animal models provide insight into the human situation .
	manualset3
231963	8	421676	7	NULL	NULL	0	NULL	human situation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the exact cascade of events that culminate into a migraine attack remains elusive , the mechanisms that underlie the manifestation of migraine pain have been better studied , and results obtained in animal models provide insight into the human situation .
	manualset3
231964	1	421677	7	NULL	NULL	0	NULL	Ultrasound mediated microbubble destruction	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound mediated microbubble destruction provides a new option for noninvasive gene transfer in heart .
	manualset3
231965	2	421677	7	NULL	NULL	0	NULL	 new option	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound mediated microbubble destruction provides a new option for noninvasive gene transfer in heart .
	manualset3
231966	3	421677	7	NULL	NULL	0	NULL	 noninvasive gene transfer	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound mediated microbubble destruction provides a new option for noninvasive gene transfer in heart .
	manualset3
231967	4	421677	7	NULL	NULL	0	NULL	heart 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultrasound mediated microbubble destruction provides a new option for noninvasive gene transfer in heart .
	manualset3
232497	1	421678	7	NULL	NULL	0	NULL	Mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in domain L that prevented the binding of CCAAT box binding activities reduced both hepatic and intestinal transcription to 30 % of control , indicating the importance of these factors in transcription .
	manualset3
232498	2	421678	7	NULL	NULL	0	NULL	domain L	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in domain L that prevented the binding of CCAAT box binding activities reduced both hepatic and intestinal transcription to 30 % of control , indicating the importance of these factors in transcription .
	manualset3
232499	3	421678	7	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in domain L that prevented the binding of CCAAT box binding activities reduced both hepatic and intestinal transcription to 30 % of control , indicating the importance of these factors in transcription .
	manualset3
232500	4	421678	7	NULL	NULL	0	NULL	CCAAT box binding activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in domain L that prevented the binding of CCAAT box binding activities reduced both hepatic and intestinal transcription to 30 % of control , indicating the importance of these factors in transcription .
	manualset3
232501	5	421678	7	NULL	NULL	0	NULL	 hepatic transcription 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in domain L that prevented the binding of CCAAT box binding activities reduced both hepatic and intestinal transcription to 30 % of control , indicating the importance of these factors in transcription .
	manualset3
232502	6	421678	7	NULL	NULL	0	NULL	intestinal transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in domain L that prevented the binding of CCAAT box binding activities reduced both hepatic and intestinal transcription to 30 % of control , indicating the importance of these factors in transcription .
	manualset3
232503	7	421678	7	NULL	NULL	0	NULL	30 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in domain L that prevented the binding of CCAAT box binding activities reduced both hepatic and intestinal transcription to 30 % of control , indicating the importance of these factors in transcription .
	manualset3
232504	8	421678	7	NULL	NULL	0	NULL	control	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in domain L that prevented the binding of CCAAT box binding activities reduced both hepatic and intestinal transcription to 30 % of control , indicating the importance of these factors in transcription .
	manualset3
232505	9	421678	7	NULL	NULL	0	NULL	factors	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in domain L that prevented the binding of CCAAT box binding activities reduced both hepatic and intestinal transcription to 30 % of control , indicating the importance of these factors in transcription .
	manualset3
232506	10	421678	7	NULL	NULL	0	NULL	transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations in domain L that prevented the binding of CCAAT box binding activities reduced both hepatic and intestinal transcription to 30 % of control , indicating the importance of these factors in transcription .
	manualset3
232507	1	421679	7	NULL	NULL	0	NULL	inferior fornix incision	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	When combined with an inferior fornix incision , the transcaruncular approach allows for continuous exposure from the frontozygomatic suture laterally to the frontoethmoidal suture medially .
	manualset3
232508	2	421679	7	NULL	NULL	0	NULL	transcaruncular approach	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	When combined with an inferior fornix incision , the transcaruncular approach allows for continuous exposure from the frontozygomatic suture laterally to the frontoethmoidal suture medially .
	manualset3
232509	3	421679	7	NULL	NULL	0	NULL	continuous exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When combined with an inferior fornix incision , the transcaruncular approach allows for continuous exposure from the frontozygomatic suture laterally to the frontoethmoidal suture medially .
	manualset3
232510	4	421679	7	NULL	NULL	0	NULL	frontozygomatic suture	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	When combined with an inferior fornix incision , the transcaruncular approach allows for continuous exposure from the frontozygomatic suture laterally to the frontoethmoidal suture medially .
	manualset3
232511	5	421679	7	NULL	NULL	0	NULL	frontoethmoidal suture	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	When combined with an inferior fornix incision , the transcaruncular approach allows for continuous exposure from the frontozygomatic suture laterally to the frontoethmoidal suture medially .
	manualset3
232512	1	421680	7	NULL	NULL	0	NULL	Diagnosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Diagnosis and therapy of acute bacterial infections of the eye ) .
	manualset3
232513	2	421680	7	NULL	NULL	0	NULL	 therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Diagnosis and therapy of acute bacterial infections of the eye ) .
	manualset3
232514	3	421680	7	NULL	NULL	0	NULL	acute bacterial infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Diagnosis and therapy of acute bacterial infections of the eye ) .
	manualset3
232515	4	421680	7	NULL	NULL	0	NULL	eye	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Diagnosis and therapy of acute bacterial infections of the eye ) .
	manualset3
232516	1	421681	7	NULL	NULL	0	NULL	normal aging population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the normal aging population , there is no evidence that ventilation limits exercise .
	manualset3
232517	2	421681	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the normal aging population , there is no evidence that ventilation limits exercise .
	manualset3
232518	3	421681	7	NULL	NULL	0	NULL	ventilation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the normal aging population , there is no evidence that ventilation limits exercise .
	manualset3
232519	4	421681	7	NULL	NULL	0	NULL	exercise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In the normal aging population , there is no evidence that ventilation limits exercise .
	manualset3
232521	1	421682	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the slopes of the relations between end-systolic wall stress and ejection fraction or mean velocity of shortening were abnormal in patients with HC ; the slope of the stress-volume trajectory during late ejection was also depressed in 12 patients with HC ( average slope 2.6 versus 5.5 kdyne/cm5/m2 , p less than 0.001 ) .
	manualset3
232522	2	421682	7	NULL	NULL	0	NULL	slopes	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the slopes of the relations between end-systolic wall stress and ejection fraction or mean velocity of shortening were abnormal in patients with HC ; the slope of the stress-volume trajectory during late ejection was also depressed in 12 patients with HC ( average slope 2.6 versus 5.5 kdyne/cm5/m2 , p less than 0.001 ) .
	manualset3
232523	3	421682	7	NULL	NULL	0	NULL	 relations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the slopes of the relations between end-systolic wall stress and ejection fraction or mean velocity of shortening were abnormal in patients with HC ; the slope of the stress-volume trajectory during late ejection was also depressed in 12 patients with HC ( average slope 2.6 versus 5.5 kdyne/cm5/m2 , p less than 0.001 ) .
	manualset3
232524	4	421682	7	NULL	NULL	0	NULL	end-systolic wall stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the slopes of the relations between end-systolic wall stress and ejection fraction or mean velocity of shortening were abnormal in patients with HC ; the slope of the stress-volume trajectory during late ejection was also depressed in 12 patients with HC ( average slope 2.6 versus 5.5 kdyne/cm5/m2 , p less than 0.001 ) .
	manualset3
232525	5	421682	7	NULL	NULL	0	NULL	ejection fraction	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the slopes of the relations between end-systolic wall stress and ejection fraction or mean velocity of shortening were abnormal in patients with HC ; the slope of the stress-volume trajectory during late ejection was also depressed in 12 patients with HC ( average slope 2.6 versus 5.5 kdyne/cm5/m2 , p less than 0.001 ) .
	manualset3
232526	6	421682	7	NULL	NULL	0	NULL	mean velocity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the slopes of the relations between end-systolic wall stress and ejection fraction or mean velocity of shortening were abnormal in patients with HC ; the slope of the stress-volume trajectory during late ejection was also depressed in 12 patients with HC ( average slope 2.6 versus 5.5 kdyne/cm5/m2 , p less than 0.001 ) .
	manualset3
232527	7	421682	7	NULL	NULL	0	NULL	shortening	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the slopes of the relations between end-systolic wall stress and ejection fraction or mean velocity of shortening were abnormal in patients with HC ; the slope of the stress-volume trajectory during late ejection was also depressed in 12 patients with HC ( average slope 2.6 versus 5.5 kdyne/cm5/m2 , p less than 0.001 ) .
	manualset3
232528	8	421682	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the slopes of the relations between end-systolic wall stress and ejection fraction or mean velocity of shortening were abnormal in patients with HC ; the slope of the stress-volume trajectory during late ejection was also depressed in 12 patients with HC ( average slope 2.6 versus 5.5 kdyne/cm5/m2 , p less than 0.001 ) .
	manualset3
232529	9	421682	7	NULL	NULL	0	NULL	HC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the slopes of the relations between end-systolic wall stress and ejection fraction or mean velocity of shortening were abnormal in patients with HC ; the slope of the stress-volume trajectory during late ejection was also depressed in 12 patients with HC ( average slope 2.6 versus 5.5 kdyne/cm5/m2 , p less than 0.001 ) .
	manualset3
232530	10	421682	7	NULL	NULL	0	NULL	slope	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the slopes of the relations between end-systolic wall stress and ejection fraction or mean velocity of shortening were abnormal in patients with HC ; the slope of the stress-volume trajectory during late ejection was also depressed in 12 patients with HC ( average slope 2.6 versus 5.5 kdyne/cm5/m2 , p less than 0.001 ) .
	manualset3
232531	11	421682	7	NULL	NULL	0	NULL	stress-volume trajectory	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the slopes of the relations between end-systolic wall stress and ejection fraction or mean velocity of shortening were abnormal in patients with HC ; the slope of the stress-volume trajectory during late ejection was also depressed in 12 patients with HC ( average slope 2.6 versus 5.5 kdyne/cm5/m2 , p less than 0.001 ) .
	manualset3
232532	12	421682	7	NULL	NULL	0	NULL	late ejection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the slopes of the relations between end-systolic wall stress and ejection fraction or mean velocity of shortening were abnormal in patients with HC ; the slope of the stress-volume trajectory during late ejection was also depressed in 12 patients with HC ( average slope 2.6 versus 5.5 kdyne/cm5/m2 , p less than 0.001 ) .
	manualset3
232533	13	421682	7	NULL	NULL	0	NULL	12 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the slopes of the relations between end-systolic wall stress and ejection fraction or mean velocity of shortening were abnormal in patients with HC ; the slope of the stress-volume trajectory during late ejection was also depressed in 12 patients with HC ( average slope 2.6 versus 5.5 kdyne/cm5/m2 , p less than 0.001 ) .
	manualset3
232534	14	421682	7	NULL	NULL	0	NULL	HC	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the slopes of the relations between end-systolic wall stress and ejection fraction or mean velocity of shortening were abnormal in patients with HC ; the slope of the stress-volume trajectory during late ejection was also depressed in 12 patients with HC ( average slope 2.6 versus 5.5 kdyne/cm5/m2 , p less than 0.001 ) .
	manualset3
232535	15	421682	7	NULL	NULL	0	NULL	average slope	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the slopes of the relations between end-systolic wall stress and ejection fraction or mean velocity of shortening were abnormal in patients with HC ; the slope of the stress-volume trajectory during late ejection was also depressed in 12 patients with HC ( average slope 2.6 versus 5.5 kdyne/cm5/m2 , p less than 0.001 ) .
	manualset3
232536	16	421682	7	NULL	NULL	0	NULL	2.6	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the slopes of the relations between end-systolic wall stress and ejection fraction or mean velocity of shortening were abnormal in patients with HC ; the slope of the stress-volume trajectory during late ejection was also depressed in 12 patients with HC ( average slope 2.6 versus 5.5 kdyne/cm5/m2 , p less than 0.001 ) .
	manualset3
232537	17	421682	7	NULL	NULL	0	NULL	 5.5 kdyne/cm5/m2	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In addition , the slopes of the relations between end-systolic wall stress and ejection fraction or mean velocity of shortening were abnormal in patients with HC ; the slope of the stress-volume trajectory during late ejection was also depressed in 12 patients with HC ( average slope 2.6 versus 5.5 kdyne/cm5/m2 , p less than 0.001 ) .
	manualset3
232538	18	421682	7	NULL	NULL	NULL	NULL	p less than 0.001	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In addition , the slopes of the relations between end-systolic wall stress and ejection fraction or mean velocity of shortening were abnormal in patients with HC ; the slope of the stress-volume trajectory during late ejection was also depressed in 12 patients with HC ( average slope 2.6 versus 5.5 kdyne/cm5/m2 , p less than 0.001 ) .
	manualset3
232540	1	421683	7	NULL	NULL	0	NULL	kinetic effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A kinetic effect of different premixing conditions on the reaction rate has been observed and attributed to the presence of NADH formed in the ` blank reaction ' between NAD and residual ethanol tightly bound to alcohol dehydrogenase .
	manualset3
232541	2	421683	7	NULL	NULL	0	NULL	premixing conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A kinetic effect of different premixing conditions on the reaction rate has been observed and attributed to the presence of NADH formed in the ` blank reaction ' between NAD and residual ethanol tightly bound to alcohol dehydrogenase .
	manualset3
232542	3	421683	7	NULL	NULL	0	NULL	reaction rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A kinetic effect of different premixing conditions on the reaction rate has been observed and attributed to the presence of NADH formed in the ` blank reaction ' between NAD and residual ethanol tightly bound to alcohol dehydrogenase .
	manualset3
232543	4	421683	7	NULL	NULL	0	NULL	NADH	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A kinetic effect of different premixing conditions on the reaction rate has been observed and attributed to the presence of NADH formed in the ` blank reaction ' between NAD and residual ethanol tightly bound to alcohol dehydrogenase .
	manualset3
232544	5	421683	7	NULL	NULL	0	NULL	 ` blank reaction '	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A kinetic effect of different premixing conditions on the reaction rate has been observed and attributed to the presence of NADH formed in the ` blank reaction ' between NAD and residual ethanol tightly bound to alcohol dehydrogenase .
	manualset3
232545	6	421683	7	NULL	NULL	0	NULL	NAD	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A kinetic effect of different premixing conditions on the reaction rate has been observed and attributed to the presence of NADH formed in the ` blank reaction ' between NAD and residual ethanol tightly bound to alcohol dehydrogenase .
	manualset3
232546	7	421683	7	NULL	NULL	0	NULL	residual ethanol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A kinetic effect of different premixing conditions on the reaction rate has been observed and attributed to the presence of NADH formed in the ` blank reaction ' between NAD and residual ethanol tightly bound to alcohol dehydrogenase .
	manualset3
232547	8	421683	7	NULL	NULL	0	NULL	alcohol dehydrogenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A kinetic effect of different premixing conditions on the reaction rate has been observed and attributed to the presence of NADH formed in the ` blank reaction ' between NAD and residual ethanol tightly bound to alcohol dehydrogenase .
	manualset3
235754	9	421683	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A kinetic effect of different premixing conditions on the reaction rate has been observed and attributed to the presence of NADH formed in the ` blank reaction ' between NAD and residual ethanol tightly bound to alcohol dehydrogenase .
	manualset3
232549	1	421684	7	NULL	NULL	0	NULL	first study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , this is the first study which reports bla ( CTX-M ) located on genomic DNA of bacteria from India .
	manualset3
232550	2	421684	7	NULL	NULL	0	NULL	bla ( CTX-M ) 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , this is the first study which reports bla ( CTX-M ) located on genomic DNA of bacteria from India .
	manualset3
232551	3	421684	7	NULL	NULL	0	NULL	genomic DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , this is the first study which reports bla ( CTX-M ) located on genomic DNA of bacteria from India .
	manualset3
232552	4	421684	7	NULL	NULL	0	NULL	 bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , this is the first study which reports bla ( CTX-M ) located on genomic DNA of bacteria from India .
	manualset3
232553	5	421684	7	NULL	NULL	0	NULL	India	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Moreover , this is the first study which reports bla ( CTX-M ) located on genomic DNA of bacteria from India .
	manualset3
232554	1	421685	7	NULL	NULL	0	NULL	vesicular transport	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter is mediated by vesicular transport involving the sorting of specialized cargo into the secretory granules ( SGs ) , thereby generating the transport vesicles ; their transport along the microtubules and eventually their signal-dependent fusion with the plasma membrane .
	manualset3
232555	2	421685	7	NULL	NULL	0	NULL	 sorting	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter is mediated by vesicular transport involving the sorting of specialized cargo into the secretory granules ( SGs ) , thereby generating the transport vesicles ; their transport along the microtubules and eventually their signal-dependent fusion with the plasma membrane .
	manualset3
232556	3	421685	7	NULL	NULL	0	NULL	specialized cargo	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter is mediated by vesicular transport involving the sorting of specialized cargo into the secretory granules ( SGs ) , thereby generating the transport vesicles ; their transport along the microtubules and eventually their signal-dependent fusion with the plasma membrane .
	manualset3
232557	4	421685	7	NULL	NULL	0	NULL	 secretory granules ( SGs )	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter is mediated by vesicular transport involving the sorting of specialized cargo into the secretory granules ( SGs ) , thereby generating the transport vesicles ; their transport along the microtubules and eventually their signal-dependent fusion with the plasma membrane .
	manualset3
232558	5	421685	7	NULL	NULL	0	NULL	 transport vesicles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter is mediated by vesicular transport involving the sorting of specialized cargo into the secretory granules ( SGs ) , thereby generating the transport vesicles ; their transport along the microtubules and eventually their signal-dependent fusion with the plasma membrane .
	manualset3
232559	6	421685	7	NULL	NULL	0	NULL	transport	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter is mediated by vesicular transport involving the sorting of specialized cargo into the secretory granules ( SGs ) , thereby generating the transport vesicles ; their transport along the microtubules and eventually their signal-dependent fusion with the plasma membrane .
	manualset3
232560	7	421685	7	NULL	NULL	0	NULL	microtubules	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter is mediated by vesicular transport involving the sorting of specialized cargo into the secretory granules ( SGs ) , thereby generating the transport vesicles ; their transport along the microtubules and eventually their signal-dependent fusion with the plasma membrane .
	manualset3
232561	8	421685	7	NULL	NULL	0	NULL	signal-dependent fusion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter is mediated by vesicular transport involving the sorting of specialized cargo into the secretory granules ( SGs ) , thereby generating the transport vesicles ; their transport along the microtubules and eventually their signal-dependent fusion with the plasma membrane .
	manualset3
232562	9	421685	7	NULL	NULL	0	NULL	plasma membrane 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter is mediated by vesicular transport involving the sorting of specialized cargo into the secretory granules ( SGs ) , thereby generating the transport vesicles ; their transport along the microtubules and eventually their signal-dependent fusion with the plasma membrane .
	manualset3
232563	1	421686	7	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study aimed to determine whether this interaction results in increased constitutive JNK activity in the absence of GSTP in GstP1/P2 ( - / - ) mice and whether such a phenomenon leads to the up-regulation of genes that are relevant to cell defense .
	manualset3
232564	2	421686	7	NULL	NULL	0	NULL	interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study aimed to determine whether this interaction results in increased constitutive JNK activity in the absence of GSTP in GstP1/P2 ( - / - ) mice and whether such a phenomenon leads to the up-regulation of genes that are relevant to cell defense .
	manualset3
232565	3	421686	7	NULL	NULL	0	NULL	constitutive JNK activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study aimed to determine whether this interaction results in increased constitutive JNK activity in the absence of GSTP in GstP1/P2 ( - / - ) mice and whether such a phenomenon leads to the up-regulation of genes that are relevant to cell defense .
	manualset3
232566	4	421686	7	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study aimed to determine whether this interaction results in increased constitutive JNK activity in the absence of GSTP in GstP1/P2 ( - / - ) mice and whether such a phenomenon leads to the up-regulation of genes that are relevant to cell defense .
	manualset3
232567	5	421686	7	NULL	NULL	0	NULL	GSTP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study aimed to determine whether this interaction results in increased constitutive JNK activity in the absence of GSTP in GstP1/P2 ( - / - ) mice and whether such a phenomenon leads to the up-regulation of genes that are relevant to cell defense .
	manualset3
232568	6	421686	7	NULL	NULL	0	NULL	GstP1/P2 ( - / - ) mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study aimed to determine whether this interaction results in increased constitutive JNK activity in the absence of GSTP in GstP1/P2 ( - / - ) mice and whether such a phenomenon leads to the up-regulation of genes that are relevant to cell defense .
	manualset3
232569	7	421686	7	NULL	NULL	0	NULL	phenomenon 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study aimed to determine whether this interaction results in increased constitutive JNK activity in the absence of GSTP in GstP1/P2 ( - / - ) mice and whether such a phenomenon leads to the up-regulation of genes that are relevant to cell defense .
	manualset3
232570	8	421686	7	NULL	NULL	0	NULL	 up-regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study aimed to determine whether this interaction results in increased constitutive JNK activity in the absence of GSTP in GstP1/P2 ( - / - ) mice and whether such a phenomenon leads to the up-regulation of genes that are relevant to cell defense .
	manualset3
232571	9	421686	7	NULL	NULL	0	NULL	genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study aimed to determine whether this interaction results in increased constitutive JNK activity in the absence of GSTP in GstP1/P2 ( - / - ) mice and whether such a phenomenon leads to the up-regulation of genes that are relevant to cell defense .
	manualset3
232572	10	421686	7	NULL	NULL	0	NULL	cell defense	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present study aimed to determine whether this interaction results in increased constitutive JNK activity in the absence of GSTP in GstP1/P2 ( - / - ) mice and whether such a phenomenon leads to the up-regulation of genes that are relevant to cell defense .
	manualset3
232573	1	421687	7	NULL	NULL	0	NULL	Scatchard analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Scatchard analysis of myosin V binding to stripped dense vesicles showed saturable binding with a K ( m ) of 10 nM .
	manualset3
232574	2	421687	7	NULL	NULL	0	NULL	myosin V binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Scatchard analysis of myosin V binding to stripped dense vesicles showed saturable binding with a K ( m ) of 10 nM .
	manualset3
232575	3	421687	7	NULL	NULL	0	NULL	stripped dense vesicles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Scatchard analysis of myosin V binding to stripped dense vesicles showed saturable binding with a K ( m ) of 10 nM .
	manualset3
232576	4	421687	7	NULL	NULL	0	NULL	saturable binding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Scatchard analysis of myosin V binding to stripped dense vesicles showed saturable binding with a K ( m ) of 10 nM .
	manualset3
232577	5	421687	7	NULL	NULL	0	NULL	K ( m )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Scatchard analysis of myosin V binding to stripped dense vesicles showed saturable binding with a K ( m ) of 10 nM .
	manualset3
232578	6	421687	7	NULL	NULL	0	NULL	10 nM 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Scatchard analysis of myosin V binding to stripped dense vesicles showed saturable binding with a K ( m ) of 10 nM .
	manualset3
232579	1	421688	7	NULL	NULL	0	NULL	Cockayne syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Cockayne syndrome is a related disorder with defective TCR and consists of two complementation groups , Cockayne syndrome ( CS ) - A and CS-B , which are caused by mutations in ERCC8 ( CSA ) and ERCC6 ( CSB ) , respectively .
	manualset3
232580	2	421688	7	NULL	NULL	0	NULL	related disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Cockayne syndrome is a related disorder with defective TCR and consists of two complementation groups , Cockayne syndrome ( CS ) - A and CS-B , which are caused by mutations in ERCC8 ( CSA ) and ERCC6 ( CSB ) , respectively .
	manualset3
232581	3	421688	7	NULL	NULL	0	NULL	defective TCR	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cockayne syndrome is a related disorder with defective TCR and consists of two complementation groups , Cockayne syndrome ( CS ) - A and CS-B , which are caused by mutations in ERCC8 ( CSA ) and ERCC6 ( CSB ) , respectively .
	manualset3
232582	4	421688	7	NULL	NULL	0	NULL	two complementation groups	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Cockayne syndrome is a related disorder with defective TCR and consists of two complementation groups , Cockayne syndrome ( CS ) - A and CS-B , which are caused by mutations in ERCC8 ( CSA ) and ERCC6 ( CSB ) , respectively .
	manualset3
232583	5	421688	7	NULL	NULL	0	NULL	Cockayne syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Cockayne syndrome is a related disorder with defective TCR and consists of two complementation groups , Cockayne syndrome ( CS ) - A and CS-B , which are caused by mutations in ERCC8 ( CSA ) and ERCC6 ( CSB ) , respectively .
	manualset3
232584	6	421688	7	NULL	NULL	NULL	NULL	( CS ) - A 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cockayne syndrome is a related disorder with defective TCR and consists of two complementation groups , Cockayne syndrome ( CS ) - A and CS-B , which are caused by mutations in ERCC8 ( CSA ) and ERCC6 ( CSB ) , respectively .
	manualset3
232585	7	421688	7	NULL	NULL	NULL	NULL	CS-B	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cockayne syndrome is a related disorder with defective TCR and consists of two complementation groups , Cockayne syndrome ( CS ) - A and CS-B , which are caused by mutations in ERCC8 ( CSA ) and ERCC6 ( CSB ) , respectively .
	manualset3
232586	8	421688	7	NULL	NULL	0	NULL	mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cockayne syndrome is a related disorder with defective TCR and consists of two complementation groups , Cockayne syndrome ( CS ) - A and CS-B , which are caused by mutations in ERCC8 ( CSA ) and ERCC6 ( CSB ) , respectively .
	manualset3
232587	9	421688	7	NULL	NULL	0	NULL	ERCC8 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Cockayne syndrome is a related disorder with defective TCR and consists of two complementation groups , Cockayne syndrome ( CS ) - A and CS-B , which are caused by mutations in ERCC8 ( CSA ) and ERCC6 ( CSB ) , respectively .
	manualset3
232588	10	421688	7	NULL	NULL	0	NULL	CSA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Cockayne syndrome is a related disorder with defective TCR and consists of two complementation groups , Cockayne syndrome ( CS ) - A and CS-B , which are caused by mutations in ERCC8 ( CSA ) and ERCC6 ( CSB ) , respectively .
	manualset3
232589	11	421688	7	NULL	NULL	0	NULL	ERCC6	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Cockayne syndrome is a related disorder with defective TCR and consists of two complementation groups , Cockayne syndrome ( CS ) - A and CS-B , which are caused by mutations in ERCC8 ( CSA ) and ERCC6 ( CSB ) , respectively .
	manualset3
232590	12	421688	7	NULL	NULL	0	NULL	CSB	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Cockayne syndrome is a related disorder with defective TCR and consists of two complementation groups , Cockayne syndrome ( CS ) - A and CS-B , which are caused by mutations in ERCC8 ( CSA ) and ERCC6 ( CSB ) , respectively .
	manualset3
232591	1	421689	7	NULL	NULL	0	NULL	complete homology	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	An apparent complete homology between bovine protein AA and protein AA from other species was apparent at positions 35-45 , providing further evidence that this is a functionally significant part of the serum protein AA ( SAA ) molecule .
	manualset3
232592	2	421689	7	NULL	NULL	0	NULL	bovine protein AA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	An apparent complete homology between bovine protein AA and protein AA from other species was apparent at positions 35-45 , providing further evidence that this is a functionally significant part of the serum protein AA ( SAA ) molecule .
	manualset3
232593	3	421689	7	NULL	NULL	0	NULL	protein AA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	An apparent complete homology between bovine protein AA and protein AA from other species was apparent at positions 35-45 , providing further evidence that this is a functionally significant part of the serum protein AA ( SAA ) molecule .
	manualset3
232594	4	421689	7	NULL	NULL	0	NULL	species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	An apparent complete homology between bovine protein AA and protein AA from other species was apparent at positions 35-45 , providing further evidence that this is a functionally significant part of the serum protein AA ( SAA ) molecule .
	manualset3
232595	5	421689	7	NULL	NULL	0	NULL	positions 35-45	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	An apparent complete homology between bovine protein AA and protein AA from other species was apparent at positions 35-45 , providing further evidence that this is a functionally significant part of the serum protein AA ( SAA ) molecule .
	manualset3
232596	6	421689	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An apparent complete homology between bovine protein AA and protein AA from other species was apparent at positions 35-45 , providing further evidence that this is a functionally significant part of the serum protein AA ( SAA ) molecule .
	manualset3
232597	7	421689	7	NULL	NULL	0	NULL	serum protein AA ( SAA ) molecule	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	An apparent complete homology between bovine protein AA and protein AA from other species was apparent at positions 35-45 , providing further evidence that this is a functionally significant part of the serum protein AA ( SAA ) molecule .
	manualset3
232598	1	421690	7	NULL	NULL	0	NULL	neurotransmitters	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The neurotransmitters expressed by neurons activated by D-fenfluramine ( 5 mg/kg , i.p. ) were identified in the hypothalamus , amygdala and bed nucleus of the stria terminalis .
	manualset3
232599	2	421690	7	NULL	NULL	0	NULL	 neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The neurotransmitters expressed by neurons activated by D-fenfluramine ( 5 mg/kg , i.p. ) were identified in the hypothalamus , amygdala and bed nucleus of the stria terminalis .
	manualset3
232600	3	421690	7	NULL	NULL	0	NULL	D-fenfluramine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The neurotransmitters expressed by neurons activated by D-fenfluramine ( 5 mg/kg , i.p. ) were identified in the hypothalamus , amygdala and bed nucleus of the stria terminalis .
	manualset3
232601	4	421690	7	NULL	NULL	0	NULL	 5 mg/kg 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The neurotransmitters expressed by neurons activated by D-fenfluramine ( 5 mg/kg , i.p. ) were identified in the hypothalamus , amygdala and bed nucleus of the stria terminalis .
	manualset3
232602	5	421690	7	NULL	NULL	0	NULL	 i.p.	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The neurotransmitters expressed by neurons activated by D-fenfluramine ( 5 mg/kg , i.p. ) were identified in the hypothalamus , amygdala and bed nucleus of the stria terminalis .
	manualset3
232603	6	421690	7	NULL	NULL	0	NULL	hypothalamus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The neurotransmitters expressed by neurons activated by D-fenfluramine ( 5 mg/kg , i.p. ) were identified in the hypothalamus , amygdala and bed nucleus of the stria terminalis .
	manualset3
232604	7	421690	7	NULL	NULL	0	NULL	amygdala	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The neurotransmitters expressed by neurons activated by D-fenfluramine ( 5 mg/kg , i.p. ) were identified in the hypothalamus , amygdala and bed nucleus of the stria terminalis .
	manualset3
232605	8	421690	7	NULL	NULL	0	NULL	bed nucleus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The neurotransmitters expressed by neurons activated by D-fenfluramine ( 5 mg/kg , i.p. ) were identified in the hypothalamus , amygdala and bed nucleus of the stria terminalis .
	manualset3
232606	9	421690	7	NULL	NULL	0	NULL	stria terminalis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The neurotransmitters expressed by neurons activated by D-fenfluramine ( 5 mg/kg , i.p. ) were identified in the hypothalamus , amygdala and bed nucleus of the stria terminalis .
	manualset3
232607	1	421691	7	NULL	NULL	0	NULL	SubAB	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We found that SubAB activated ERK and Akt , and inhibition of individual kinases enhanced SubAB-triggered apoptosis .
	manualset3
232608	2	421691	7	NULL	NULL	0	NULL	ERK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We found that SubAB activated ERK and Akt , and inhibition of individual kinases enhanced SubAB-triggered apoptosis .
	manualset3
232609	3	421691	7	NULL	NULL	0	NULL	Akt 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We found that SubAB activated ERK and Akt , and inhibition of individual kinases enhanced SubAB-triggered apoptosis .
	manualset3
232610	4	421691	7	NULL	NULL	0	NULL	inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We found that SubAB activated ERK and Akt , and inhibition of individual kinases enhanced SubAB-triggered apoptosis .
	manualset3
232611	5	421691	7	NULL	NULL	0	NULL	 individual kinases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We found that SubAB activated ERK and Akt , and inhibition of individual kinases enhanced SubAB-triggered apoptosis .
	manualset3
232612	6	421691	7	NULL	NULL	0	NULL	SubAB-triggered apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We found that SubAB activated ERK and Akt , and inhibition of individual kinases enhanced SubAB-triggered apoptosis .
	manualset3
232613	1	421692	7	NULL	NULL	0	NULL	Cerebral abscess	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Cerebral abscess presenting as larceny .
	manualset3
232614	2	421692	7	NULL	NULL	0	NULL	 larceny	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Cerebral abscess presenting as larceny .
	manualset3
232615	1	421693	7	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The therapy of prostate cancer has changed little over the past 10 years .
	manualset3
232616	2	421693	7	NULL	NULL	0	NULL	prostate cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The therapy of prostate cancer has changed little over the past 10 years .
	manualset3
232617	3	421693	7	NULL	NULL	0	NULL	 10 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The therapy of prostate cancer has changed little over the past 10 years .
	manualset3
232618	1	421694	7	NULL	NULL	0	NULL	taxanes	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Like taxanes , eribulin inhibits microtubule function .
	manualset3
232619	2	421694	7	NULL	NULL	0	NULL	eribulin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Like taxanes , eribulin inhibits microtubule function .
	manualset3
232620	3	421694	7	NULL	NULL	0	NULL	microtubule function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Like taxanes , eribulin inhibits microtubule function .
	manualset3
232621	1	421695	7	NULL	NULL	0	NULL	antidepressant drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Many antidepressant drugs , when administered chronically to rats , have been shown to produce decreases in the density of beta adrenergic receptors in the central nervous system .
	manualset3
232622	2	421695	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Many antidepressant drugs , when administered chronically to rats , have been shown to produce decreases in the density of beta adrenergic receptors in the central nervous system .
	manualset3
232623	3	421695	7	NULL	NULL	0	NULL	 density 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Many antidepressant drugs , when administered chronically to rats , have been shown to produce decreases in the density of beta adrenergic receptors in the central nervous system .
	manualset3
232624	4	421695	7	NULL	NULL	0	NULL	beta adrenergic receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Many antidepressant drugs , when administered chronically to rats , have been shown to produce decreases in the density of beta adrenergic receptors in the central nervous system .
	manualset3
232625	5	421695	7	NULL	NULL	0	NULL	central nervous system 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Many antidepressant drugs , when administered chronically to rats , have been shown to produce decreases in the density of beta adrenergic receptors in the central nervous system .
	manualset3
232626	1	421696	7	NULL	NULL	0	NULL	Differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	( Differences in absenteeism due to illness among women physicians and nurses in outpatient clinics and hospitals ) .
	manualset3
232627	2	421696	7	NULL	NULL	0	NULL	absenteeism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Differences in absenteeism due to illness among women physicians and nurses in outpatient clinics and hospitals ) .
	manualset3
232628	3	421696	7	NULL	NULL	0	NULL	 illness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Differences in absenteeism due to illness among women physicians and nurses in outpatient clinics and hospitals ) .
	manualset3
232629	4	421696	7	NULL	NULL	0	NULL	women physicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Differences in absenteeism due to illness among women physicians and nurses in outpatient clinics and hospitals ) .
	manualset3
232630	5	421696	7	NULL	NULL	0	NULL	nurses	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Differences in absenteeism due to illness among women physicians and nurses in outpatient clinics and hospitals ) .
	manualset3
232631	6	421696	7	NULL	NULL	0	NULL	outpatient clinics	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( Differences in absenteeism due to illness among women physicians and nurses in outpatient clinics and hospitals ) .
	manualset3
232632	7	421696	7	NULL	NULL	0	NULL	hospitals	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( Differences in absenteeism due to illness among women physicians and nurses in outpatient clinics and hospitals ) .
	manualset3
232634	1	421697	7	NULL	NULL	0	NULL	multi-joints coordination motor mode	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An apparent multi-joints coordination motor mode was employed to compensate the influences of loading , however , their contributions are different ; hip , knee joints and torso pitch made dominant contributions to the compensation while ankle joints made minor .
	manualset3
232635	2	421697	7	NULL	NULL	0	NULL	loading	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An apparent multi-joints coordination motor mode was employed to compensate the influences of loading , however , their contributions are different ; hip , knee joints and torso pitch made dominant contributions to the compensation while ankle joints made minor .
	manualset3
232636	3	421697	7	NULL	NULL	0	NULL	contributions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An apparent multi-joints coordination motor mode was employed to compensate the influences of loading , however , their contributions are different ; hip , knee joints and torso pitch made dominant contributions to the compensation while ankle joints made minor .
	manualset3
232637	4	421697	7	NULL	NULL	0	NULL	hip	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An apparent multi-joints coordination motor mode was employed to compensate the influences of loading , however , their contributions are different ; hip , knee joints and torso pitch made dominant contributions to the compensation while ankle joints made minor .
	manualset3
232638	5	421697	7	NULL	NULL	0	NULL	knee joints	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An apparent multi-joints coordination motor mode was employed to compensate the influences of loading , however , their contributions are different ; hip , knee joints and torso pitch made dominant contributions to the compensation while ankle joints made minor .
	manualset3
232639	6	421697	7	NULL	NULL	0	NULL	torso pitch	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An apparent multi-joints coordination motor mode was employed to compensate the influences of loading , however , their contributions are different ; hip , knee joints and torso pitch made dominant contributions to the compensation while ankle joints made minor .
	manualset3
232640	7	421697	7	NULL	NULL	0	NULL	dominant contributions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An apparent multi-joints coordination motor mode was employed to compensate the influences of loading , however , their contributions are different ; hip , knee joints and torso pitch made dominant contributions to the compensation while ankle joints made minor .
	manualset3
232641	8	421697	7	NULL	NULL	0	NULL	 compensation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An apparent multi-joints coordination motor mode was employed to compensate the influences of loading , however , their contributions are different ; hip , knee joints and torso pitch made dominant contributions to the compensation while ankle joints made minor .
	manualset3
232642	9	421697	7	NULL	NULL	0	NULL	ankle joints 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An apparent multi-joints coordination motor mode was employed to compensate the influences of loading , however , their contributions are different ; hip , knee joints and torso pitch made dominant contributions to the compensation while ankle joints made minor .
	manualset3
232643	1	421698	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Further studies are needed to determine the safety and effectiveness of sirolimus-eluting stents in patients with more complex coronary artery lesions .
	manualset3
232644	2	421698	7	NULL	NULL	0	NULL	safety	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further studies are needed to determine the safety and effectiveness of sirolimus-eluting stents in patients with more complex coronary artery lesions .
	manualset3
232645	3	421698	7	NULL	NULL	0	NULL	sirolimus-eluting stents	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Further studies are needed to determine the safety and effectiveness of sirolimus-eluting stents in patients with more complex coronary artery lesions .
	manualset3
232646	4	421698	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Further studies are needed to determine the safety and effectiveness of sirolimus-eluting stents in patients with more complex coronary artery lesions .
	manualset3
232647	5	421698	7	NULL	NULL	0	NULL	complex coronary artery lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Further studies are needed to determine the safety and effectiveness of sirolimus-eluting stents in patients with more complex coronary artery lesions .
	manualset3
232648	1	421699	7	NULL	NULL	0	NULL	Pagurus criniticornis 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pagurus criniticornis showed high activity not influenced by day/night conditions during the entire observed period .
	manualset3
232649	2	421699	7	NULL	NULL	0	NULL	high activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pagurus criniticornis showed high activity not influenced by day/night conditions during the entire observed period .
	manualset3
232650	3	421699	7	NULL	NULL	0	NULL	day/night conditions	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Pagurus criniticornis showed high activity not influenced by day/night conditions during the entire observed period .
	manualset3
232651	4	421699	7	NULL	NULL	0	NULL	observed period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Pagurus criniticornis showed high activity not influenced by day/night conditions during the entire observed period .
	manualset3
232652	1	421700	7	NULL	NULL	0	NULL	Intravenous administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous administration of TB ( 50 mg/kg ) caused a decrease in the urinary excretion rate of SMZ but an increase in the unbound concentration of SMZ in plasma .
	manualset3
232653	2	421700	7	NULL	NULL	0	NULL	TB	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous administration of TB ( 50 mg/kg ) caused a decrease in the urinary excretion rate of SMZ but an increase in the unbound concentration of SMZ in plasma .
	manualset3
232654	3	421700	7	NULL	NULL	0	NULL	50 mg/kg	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous administration of TB ( 50 mg/kg ) caused a decrease in the urinary excretion rate of SMZ but an increase in the unbound concentration of SMZ in plasma .
	manualset3
232655	4	421700	7	NULL	NULL	0	NULL	urinary excretion rate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous administration of TB ( 50 mg/kg ) caused a decrease in the urinary excretion rate of SMZ but an increase in the unbound concentration of SMZ in plasma .
	manualset3
232656	5	421700	7	NULL	NULL	0	NULL	SMZ	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous administration of TB ( 50 mg/kg ) caused a decrease in the urinary excretion rate of SMZ but an increase in the unbound concentration of SMZ in plasma .
	manualset3
232657	6	421700	7	NULL	NULL	0	NULL	unbound concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous administration of TB ( 50 mg/kg ) caused a decrease in the urinary excretion rate of SMZ but an increase in the unbound concentration of SMZ in plasma .
	manualset3
232658	7	421700	7	NULL	NULL	0	NULL	SMZ	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous administration of TB ( 50 mg/kg ) caused a decrease in the urinary excretion rate of SMZ but an increase in the unbound concentration of SMZ in plasma .
	manualset3
232659	8	421700	7	NULL	NULL	0	NULL	 plasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous administration of TB ( 50 mg/kg ) caused a decrease in the urinary excretion rate of SMZ but an increase in the unbound concentration of SMZ in plasma .
	manualset3
232660	1	421701	7	NULL	NULL	0	NULL	dRGII administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In line with this , we showed that dRGII administration was not effective in decreasing tibia or kidney Pb levels in rats .
	manualset3
232661	2	421701	7	NULL	NULL	0	NULL	tibia	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In line with this , we showed that dRGII administration was not effective in decreasing tibia or kidney Pb levels in rats .
	manualset3
232662	3	421701	7	NULL	NULL	0	NULL	kidney Pb levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In line with this , we showed that dRGII administration was not effective in decreasing tibia or kidney Pb levels in rats .
	manualset3
232663	4	421701	7	NULL	NULL	0	NULL	rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In line with this , we showed that dRGII administration was not effective in decreasing tibia or kidney Pb levels in rats .
	manualset3
232664	1	421702	7	NULL	NULL	0	NULL	structural analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural analysis of neutral glycolipids and gangliosides of the SV40 transformed Balb/c3T3 cells ( SV3T3 cells ) and concanavalin A-selected SV3T3 revertant cells , both compared with untransformed Balb/c3T3 cells , has shown : ( i ) a content of neutral glycolipids in revertant cells near to that found in the untransformed parental cells ; ( ii ) a similar decrease of the higher gangliosides in transformed and revertant cells ; ( iii ) a content of ganglioside GM3 in revertant cells much higher than that found in both SV3T3 and untransformed Balb/3T3 cells .
	manualset3
232665	2	421702	7	NULL	NULL	0	NULL	neutral glycolipids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural analysis of neutral glycolipids and gangliosides of the SV40 transformed Balb/c3T3 cells ( SV3T3 cells ) and concanavalin A-selected SV3T3 revertant cells , both compared with untransformed Balb/c3T3 cells , has shown : ( i ) a content of neutral glycolipids in revertant cells near to that found in the untransformed parental cells ; ( ii ) a similar decrease of the higher gangliosides in transformed and revertant cells ; ( iii ) a content of ganglioside GM3 in revertant cells much higher than that found in both SV3T3 and untransformed Balb/3T3 cells .
	manualset3
232666	3	421702	7	NULL	NULL	0	NULL	gangliosides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural analysis of neutral glycolipids and gangliosides of the SV40 transformed Balb/c3T3 cells ( SV3T3 cells ) and concanavalin A-selected SV3T3 revertant cells , both compared with untransformed Balb/c3T3 cells , has shown : ( i ) a content of neutral glycolipids in revertant cells near to that found in the untransformed parental cells ; ( ii ) a similar decrease of the higher gangliosides in transformed and revertant cells ; ( iii ) a content of ganglioside GM3 in revertant cells much higher than that found in both SV3T3 and untransformed Balb/3T3 cells .
	manualset3
232667	4	421702	7	NULL	NULL	0	NULL	SV40 transformed Balb/c3T3 cells ( SV3T3 cells )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural analysis of neutral glycolipids and gangliosides of the SV40 transformed Balb/c3T3 cells ( SV3T3 cells ) and concanavalin A-selected SV3T3 revertant cells , both compared with untransformed Balb/c3T3 cells , has shown : ( i ) a content of neutral glycolipids in revertant cells near to that found in the untransformed parental cells ; ( ii ) a similar decrease of the higher gangliosides in transformed and revertant cells ; ( iii ) a content of ganglioside GM3 in revertant cells much higher than that found in both SV3T3 and untransformed Balb/3T3 cells .
	manualset3
232668	5	421702	7	NULL	NULL	0	NULL	concanavalin A-selected SV3T3 revertant cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural analysis of neutral glycolipids and gangliosides of the SV40 transformed Balb/c3T3 cells ( SV3T3 cells ) and concanavalin A-selected SV3T3 revertant cells , both compared with untransformed Balb/c3T3 cells , has shown : ( i ) a content of neutral glycolipids in revertant cells near to that found in the untransformed parental cells ; ( ii ) a similar decrease of the higher gangliosides in transformed and revertant cells ; ( iii ) a content of ganglioside GM3 in revertant cells much higher than that found in both SV3T3 and untransformed Balb/3T3 cells .
	manualset3
232669	6	421702	7	NULL	NULL	0	NULL	untransformed Balb/c3T3 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural analysis of neutral glycolipids and gangliosides of the SV40 transformed Balb/c3T3 cells ( SV3T3 cells ) and concanavalin A-selected SV3T3 revertant cells , both compared with untransformed Balb/c3T3 cells , has shown : ( i ) a content of neutral glycolipids in revertant cells near to that found in the untransformed parental cells ; ( ii ) a similar decrease of the higher gangliosides in transformed and revertant cells ; ( iii ) a content of ganglioside GM3 in revertant cells much higher than that found in both SV3T3 and untransformed Balb/3T3 cells .
	manualset3
232670	7	421702	7	NULL	NULL	0	NULL	content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural analysis of neutral glycolipids and gangliosides of the SV40 transformed Balb/c3T3 cells ( SV3T3 cells ) and concanavalin A-selected SV3T3 revertant cells , both compared with untransformed Balb/c3T3 cells , has shown : ( i ) a content of neutral glycolipids in revertant cells near to that found in the untransformed parental cells ; ( ii ) a similar decrease of the higher gangliosides in transformed and revertant cells ; ( iii ) a content of ganglioside GM3 in revertant cells much higher than that found in both SV3T3 and untransformed Balb/3T3 cells .
	manualset3
232671	8	421702	7	NULL	NULL	0	NULL	neutral glycolipids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural analysis of neutral glycolipids and gangliosides of the SV40 transformed Balb/c3T3 cells ( SV3T3 cells ) and concanavalin A-selected SV3T3 revertant cells , both compared with untransformed Balb/c3T3 cells , has shown : ( i ) a content of neutral glycolipids in revertant cells near to that found in the untransformed parental cells ; ( ii ) a similar decrease of the higher gangliosides in transformed and revertant cells ; ( iii ) a content of ganglioside GM3 in revertant cells much higher than that found in both SV3T3 and untransformed Balb/3T3 cells .
	manualset3
232672	9	421702	7	NULL	NULL	0	NULL	revertant cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural analysis of neutral glycolipids and gangliosides of the SV40 transformed Balb/c3T3 cells ( SV3T3 cells ) and concanavalin A-selected SV3T3 revertant cells , both compared with untransformed Balb/c3T3 cells , has shown : ( i ) a content of neutral glycolipids in revertant cells near to that found in the untransformed parental cells ; ( ii ) a similar decrease of the higher gangliosides in transformed and revertant cells ; ( iii ) a content of ganglioside GM3 in revertant cells much higher than that found in both SV3T3 and untransformed Balb/3T3 cells .
	manualset3
232673	10	421702	7	NULL	NULL	0	NULL	untransformed parental cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural analysis of neutral glycolipids and gangliosides of the SV40 transformed Balb/c3T3 cells ( SV3T3 cells ) and concanavalin A-selected SV3T3 revertant cells , both compared with untransformed Balb/c3T3 cells , has shown : ( i ) a content of neutral glycolipids in revertant cells near to that found in the untransformed parental cells ; ( ii ) a similar decrease of the higher gangliosides in transformed and revertant cells ; ( iii ) a content of ganglioside GM3 in revertant cells much higher than that found in both SV3T3 and untransformed Balb/3T3 cells .
	manualset3
232674	11	421702	7	NULL	NULL	0	NULL	 decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural analysis of neutral glycolipids and gangliosides of the SV40 transformed Balb/c3T3 cells ( SV3T3 cells ) and concanavalin A-selected SV3T3 revertant cells , both compared with untransformed Balb/c3T3 cells , has shown : ( i ) a content of neutral glycolipids in revertant cells near to that found in the untransformed parental cells ; ( ii ) a similar decrease of the higher gangliosides in transformed and revertant cells ; ( iii ) a content of ganglioside GM3 in revertant cells much higher than that found in both SV3T3 and untransformed Balb/3T3 cells .
	manualset3
232675	12	421702	7	NULL	NULL	0	NULL	higher gangliosides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural analysis of neutral glycolipids and gangliosides of the SV40 transformed Balb/c3T3 cells ( SV3T3 cells ) and concanavalin A-selected SV3T3 revertant cells , both compared with untransformed Balb/c3T3 cells , has shown : ( i ) a content of neutral glycolipids in revertant cells near to that found in the untransformed parental cells ; ( ii ) a similar decrease of the higher gangliosides in transformed and revertant cells ; ( iii ) a content of ganglioside GM3 in revertant cells much higher than that found in both SV3T3 and untransformed Balb/3T3 cells .
	manualset3
232676	13	421702	7	NULL	NULL	0	NULL	revertant cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural analysis of neutral glycolipids and gangliosides of the SV40 transformed Balb/c3T3 cells ( SV3T3 cells ) and concanavalin A-selected SV3T3 revertant cells , both compared with untransformed Balb/c3T3 cells , has shown : ( i ) a content of neutral glycolipids in revertant cells near to that found in the untransformed parental cells ; ( ii ) a similar decrease of the higher gangliosides in transformed and revertant cells ; ( iii ) a content of ganglioside GM3 in revertant cells much higher than that found in both SV3T3 and untransformed Balb/3T3 cells .
	manualset3
232677	14	421702	7	NULL	NULL	0	NULL	content 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural analysis of neutral glycolipids and gangliosides of the SV40 transformed Balb/c3T3 cells ( SV3T3 cells ) and concanavalin A-selected SV3T3 revertant cells , both compared with untransformed Balb/c3T3 cells , has shown : ( i ) a content of neutral glycolipids in revertant cells near to that found in the untransformed parental cells ; ( ii ) a similar decrease of the higher gangliosides in transformed and revertant cells ; ( iii ) a content of ganglioside GM3 in revertant cells much higher than that found in both SV3T3 and untransformed Balb/3T3 cells .
	manualset3
232678	15	421702	7	NULL	NULL	0	NULL	ganglioside GM3	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural analysis of neutral glycolipids and gangliosides of the SV40 transformed Balb/c3T3 cells ( SV3T3 cells ) and concanavalin A-selected SV3T3 revertant cells , both compared with untransformed Balb/c3T3 cells , has shown : ( i ) a content of neutral glycolipids in revertant cells near to that found in the untransformed parental cells ; ( ii ) a similar decrease of the higher gangliosides in transformed and revertant cells ; ( iii ) a content of ganglioside GM3 in revertant cells much higher than that found in both SV3T3 and untransformed Balb/3T3 cells .
	manualset3
232679	16	421702	7	NULL	NULL	0	NULL	revertant cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural analysis of neutral glycolipids and gangliosides of the SV40 transformed Balb/c3T3 cells ( SV3T3 cells ) and concanavalin A-selected SV3T3 revertant cells , both compared with untransformed Balb/c3T3 cells , has shown : ( i ) a content of neutral glycolipids in revertant cells near to that found in the untransformed parental cells ; ( ii ) a similar decrease of the higher gangliosides in transformed and revertant cells ; ( iii ) a content of ganglioside GM3 in revertant cells much higher than that found in both SV3T3 and untransformed Balb/3T3 cells .
	manualset3
232680	17	421702	7	NULL	NULL	0	NULL	SV3T3 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural analysis of neutral glycolipids and gangliosides of the SV40 transformed Balb/c3T3 cells ( SV3T3 cells ) and concanavalin A-selected SV3T3 revertant cells , both compared with untransformed Balb/c3T3 cells , has shown : ( i ) a content of neutral glycolipids in revertant cells near to that found in the untransformed parental cells ; ( ii ) a similar decrease of the higher gangliosides in transformed and revertant cells ; ( iii ) a content of ganglioside GM3 in revertant cells much higher than that found in both SV3T3 and untransformed Balb/3T3 cells .
	manualset3
232681	18	421702	7	NULL	NULL	0	NULL	untransformed Balb/3T3 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The structural analysis of neutral glycolipids and gangliosides of the SV40 transformed Balb/c3T3 cells ( SV3T3 cells ) and concanavalin A-selected SV3T3 revertant cells , both compared with untransformed Balb/c3T3 cells , has shown : ( i ) a content of neutral glycolipids in revertant cells near to that found in the untransformed parental cells ; ( ii ) a similar decrease of the higher gangliosides in transformed and revertant cells ; ( iii ) a content of ganglioside GM3 in revertant cells much higher than that found in both SV3T3 and untransformed Balb/3T3 cells .
	manualset3
232682	1	421703	7	NULL	NULL	0	NULL	Toxicosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicosis in dairy cattle exposed to poison hemlock ( Conium maculatum ) in hay : isolation of Conium alkaloids in plants , hay , and urine .
	manualset3
232683	2	421703	7	NULL	NULL	0	NULL	dairy cattle	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicosis in dairy cattle exposed to poison hemlock ( Conium maculatum ) in hay : isolation of Conium alkaloids in plants , hay , and urine .
	manualset3
232685	3	421703	7	NULL	NULL	0	NULL	poison hemlock ( Conium maculatum )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicosis in dairy cattle exposed to poison hemlock ( Conium maculatum ) in hay : isolation of Conium alkaloids in plants , hay , and urine .
	manualset3
232686	4	421703	7	NULL	NULL	NULL	NULL	hay	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Toxicosis in dairy cattle exposed to poison hemlock ( Conium maculatum ) in hay : isolation of Conium alkaloids in plants , hay , and urine .
	manualset3
232687	5	421703	7	NULL	NULL	0	NULL	isolation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicosis in dairy cattle exposed to poison hemlock ( Conium maculatum ) in hay : isolation of Conium alkaloids in plants , hay , and urine .
	manualset3
232688	6	421703	7	NULL	NULL	0	NULL	Conium alkaloids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicosis in dairy cattle exposed to poison hemlock ( Conium maculatum ) in hay : isolation of Conium alkaloids in plants , hay , and urine .
	manualset3
232689	7	421703	7	NULL	NULL	0	NULL	 plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicosis in dairy cattle exposed to poison hemlock ( Conium maculatum ) in hay : isolation of Conium alkaloids in plants , hay , and urine .
	manualset3
232690	8	421703	7	NULL	NULL	0	NULL	hay	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicosis in dairy cattle exposed to poison hemlock ( Conium maculatum ) in hay : isolation of Conium alkaloids in plants , hay , and urine .
	manualset3
232691	9	421703	7	NULL	NULL	0	NULL	 urine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Toxicosis in dairy cattle exposed to poison hemlock ( Conium maculatum ) in hay : isolation of Conium alkaloids in plants , hay , and urine .
	manualset3
232853	1	421704	7	NULL	NULL	NULL	NULL	second region	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A second region , downstream of the activator and possibly located between positions -400 and -157 bp , inhibited the UCP promoter in CHO cells .
	manualset3
232854	2	421704	7	NULL	NULL	0	NULL	activator	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A second region , downstream of the activator and possibly located between positions -400 and -157 bp , inhibited the UCP promoter in CHO cells .
	manualset3
232855	3	421704	7	NULL	NULL	NULL	NULL	positions -400 and -157 bp	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A second region , downstream of the activator and possibly located between positions -400 and -157 bp , inhibited the UCP promoter in CHO cells .
	manualset3
232856	4	421704	7	NULL	NULL	0	NULL	UCP promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A second region , downstream of the activator and possibly located between positions -400 and -157 bp , inhibited the UCP promoter in CHO cells .
	manualset3
232857	5	421704	7	NULL	NULL	0	NULL	CHO cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A second region , downstream of the activator and possibly located between positions -400 and -157 bp , inhibited the UCP promoter in CHO cells .
	manualset3
232858	6	421704	7	NULL	NULL	0	NULL	downstream 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A second region , downstream of the activator and possibly located between positions -400 and -157 bp , inhibited the UCP promoter in CHO cells .
	manualset3
232859	1	421705	7	NULL	NULL	0	NULL	legal research method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( The legal research method ; an approach to enhance nursing science ) .
	manualset3
232860	2	421705	7	NULL	NULL	0	NULL	approach	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The legal research method ; an approach to enhance nursing science ) .
	manualset3
232861	3	421705	7	NULL	NULL	0	NULL	nursing science	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( The legal research method ; an approach to enhance nursing science ) .
	manualset3
232862	1	421706	7	NULL	NULL	0	NULL	appeal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An appeal to professional conscience is no guarantee that morally defensible decisions will be arrived at .
	manualset3
232863	2	421706	7	NULL	NULL	0	NULL	professional conscience	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	An appeal to professional conscience is no guarantee that morally defensible decisions will be arrived at .
	manualset3
232864	3	421706	7	NULL	NULL	0	NULL	no guarantee	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An appeal to professional conscience is no guarantee that morally defensible decisions will be arrived at .
	manualset3
232865	4	421706	7	NULL	NULL	0	NULL	defensible decisions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An appeal to professional conscience is no guarantee that morally defensible decisions will be arrived at .
	manualset3
232866	1	421707	7	NULL	NULL	0	NULL	Recent studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies have correlated the unsuccessful outcome of regenerative therapies with poor cell viability after cryopreservation .
	manualset3
232867	2	421707	7	NULL	NULL	0	NULL	unsuccessful outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies have correlated the unsuccessful outcome of regenerative therapies with poor cell viability after cryopreservation .
	manualset3
232868	3	421707	7	NULL	NULL	0	NULL	regenerative therapies 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies have correlated the unsuccessful outcome of regenerative therapies with poor cell viability after cryopreservation .
	manualset3
232869	4	421707	7	NULL	NULL	0	NULL	poor cell viability 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies have correlated the unsuccessful outcome of regenerative therapies with poor cell viability after cryopreservation .
	manualset3
232870	5	421707	7	NULL	NULL	0	NULL	cryopreservation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Recent studies have correlated the unsuccessful outcome of regenerative therapies with poor cell viability after cryopreservation .
	manualset3
232871	1	421708	7	NULL	NULL	0	NULL	Criteria of optimum	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Criteria of optimum '' are covered in this first communication .
	manualset3
232872	2	421708	7	NULL	NULL	0	NULL	 first communication	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	`` Criteria of optimum '' are covered in this first communication .
	manualset3
232873	1	421709	7	NULL	NULL	0	NULL	Plasmid pLdhA48XI	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasmid pLdhA48XI was linearized prior to transformation in order to facilitate integration into the pyrG gene used for selection .
	manualset3
232874	2	421709	7	NULL	NULL	0	NULL	transformation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasmid pLdhA48XI was linearized prior to transformation in order to facilitate integration into the pyrG gene used for selection .
	manualset3
232875	3	421709	7	NULL	NULL	0	NULL	 integration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasmid pLdhA48XI was linearized prior to transformation in order to facilitate integration into the pyrG gene used for selection .
	manualset3
232876	4	421709	7	NULL	NULL	0	NULL	 pyrG gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasmid pLdhA48XI was linearized prior to transformation in order to facilitate integration into the pyrG gene used for selection .
	manualset3
232877	5	421709	7	NULL	NULL	0	NULL	 selection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Plasmid pLdhA48XI was linearized prior to transformation in order to facilitate integration into the pyrG gene used for selection .
	manualset3
232878	1	421710	7	NULL	NULL	0	NULL	 current study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the current study , we attempted to follow-up these findings in a sample from the UK , the Depression Case Control ( DeCC ) sample consisting of 1 , 196 cases and 842 screened controls , phenotyped using exactly the same methods as the MP-GSK sample .
	manualset3
232879	2	421710	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the current study , we attempted to follow-up these findings in a sample from the UK , the Depression Case Control ( DeCC ) sample consisting of 1 , 196 cases and 842 screened controls , phenotyped using exactly the same methods as the MP-GSK sample .
	manualset3
232880	3	421710	7	NULL	NULL	0	NULL	sample	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the current study , we attempted to follow-up these findings in a sample from the UK , the Depression Case Control ( DeCC ) sample consisting of 1 , 196 cases and 842 screened controls , phenotyped using exactly the same methods as the MP-GSK sample .
	manualset3
232881	4	421710	7	NULL	NULL	0	NULL	UK	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the current study , we attempted to follow-up these findings in a sample from the UK , the Depression Case Control ( DeCC ) sample consisting of 1 , 196 cases and 842 screened controls , phenotyped using exactly the same methods as the MP-GSK sample .
	manualset3
232882	5	421710	7	NULL	NULL	0	NULL	Depression Case Control ( DeCC ) sample	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the current study , we attempted to follow-up these findings in a sample from the UK , the Depression Case Control ( DeCC ) sample consisting of 1 , 196 cases and 842 screened controls , phenotyped using exactly the same methods as the MP-GSK sample .
	manualset3
232884	7	421710	7	NULL	NULL	NULL	NULL	1 , 196 cases	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Within the current study , we attempted to follow-up these findings in a sample from the UK , the Depression Case Control ( DeCC ) sample consisting of 1 , 196 cases and 842 screened controls , phenotyped using exactly the same methods as the MP-GSK sample .
	manualset3
232885	8	421710	7	NULL	NULL	0	NULL	842 screened controls 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the current study , we attempted to follow-up these findings in a sample from the UK , the Depression Case Control ( DeCC ) sample consisting of 1 , 196 cases and 842 screened controls , phenotyped using exactly the same methods as the MP-GSK sample .
	manualset3
232886	9	421710	7	NULL	NULL	0	NULL	methods 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the current study , we attempted to follow-up these findings in a sample from the UK , the Depression Case Control ( DeCC ) sample consisting of 1 , 196 cases and 842 screened controls , phenotyped using exactly the same methods as the MP-GSK sample .
	manualset3
232887	10	421710	7	NULL	NULL	0	NULL	MP-GSK sample	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Within the current study , we attempted to follow-up these findings in a sample from the UK , the Depression Case Control ( DeCC ) sample consisting of 1 , 196 cases and 842 screened controls , phenotyped using exactly the same methods as the MP-GSK sample .
	manualset3
232888	1	421711	7	NULL	NULL	0	NULL	Fluorescence resonance energy transfer ( FRET ) - analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescence resonance energy transfer ( FRET ) - analysis in Huh7 hepatoma cells , which were cotransfected with CD95-YFP/CD95-CFP revealed that stimulation of these cells with CD95 ligand , proapoptotic bile acids or hyperosmolarity resulted within 30 min in an intracellular FRET-signal , suggestive for CD95/CD95-oligomerization .
	manualset3
232889	2	421711	7	NULL	NULL	0	NULL	Huh7 hepatoma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescence resonance energy transfer ( FRET ) - analysis in Huh7 hepatoma cells , which were cotransfected with CD95-YFP/CD95-CFP revealed that stimulation of these cells with CD95 ligand , proapoptotic bile acids or hyperosmolarity resulted within 30 min in an intracellular FRET-signal , suggestive for CD95/CD95-oligomerization .
	manualset3
232890	3	421711	7	NULL	NULL	0	NULL	CD95-YFP/CD95-CFP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescence resonance energy transfer ( FRET ) - analysis in Huh7 hepatoma cells , which were cotransfected with CD95-YFP/CD95-CFP revealed that stimulation of these cells with CD95 ligand , proapoptotic bile acids or hyperosmolarity resulted within 30 min in an intracellular FRET-signal , suggestive for CD95/CD95-oligomerization .
	manualset3
232891	4	421711	7	NULL	NULL	0	NULL	stimulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescence resonance energy transfer ( FRET ) - analysis in Huh7 hepatoma cells , which were cotransfected with CD95-YFP/CD95-CFP revealed that stimulation of these cells with CD95 ligand , proapoptotic bile acids or hyperosmolarity resulted within 30 min in an intracellular FRET-signal , suggestive for CD95/CD95-oligomerization .
	manualset3
232892	5	421711	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescence resonance energy transfer ( FRET ) - analysis in Huh7 hepatoma cells , which were cotransfected with CD95-YFP/CD95-CFP revealed that stimulation of these cells with CD95 ligand , proapoptotic bile acids or hyperosmolarity resulted within 30 min in an intracellular FRET-signal , suggestive for CD95/CD95-oligomerization .
	manualset3
232893	6	421711	7	NULL	NULL	0	NULL	CD95 ligand	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescence resonance energy transfer ( FRET ) - analysis in Huh7 hepatoma cells , which were cotransfected with CD95-YFP/CD95-CFP revealed that stimulation of these cells with CD95 ligand , proapoptotic bile acids or hyperosmolarity resulted within 30 min in an intracellular FRET-signal , suggestive for CD95/CD95-oligomerization .
	manualset3
232894	7	421711	7	NULL	NULL	0	NULL	proapoptotic bile acids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescence resonance energy transfer ( FRET ) - analysis in Huh7 hepatoma cells , which were cotransfected with CD95-YFP/CD95-CFP revealed that stimulation of these cells with CD95 ligand , proapoptotic bile acids or hyperosmolarity resulted within 30 min in an intracellular FRET-signal , suggestive for CD95/CD95-oligomerization .
	manualset3
232895	8	421711	7	NULL	NULL	0	NULL	hyperosmolarity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescence resonance energy transfer ( FRET ) - analysis in Huh7 hepatoma cells , which were cotransfected with CD95-YFP/CD95-CFP revealed that stimulation of these cells with CD95 ligand , proapoptotic bile acids or hyperosmolarity resulted within 30 min in an intracellular FRET-signal , suggestive for CD95/CD95-oligomerization .
	manualset3
232896	9	421711	7	NULL	NULL	0	NULL	30 min 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescence resonance energy transfer ( FRET ) - analysis in Huh7 hepatoma cells , which were cotransfected with CD95-YFP/CD95-CFP revealed that stimulation of these cells with CD95 ligand , proapoptotic bile acids or hyperosmolarity resulted within 30 min in an intracellular FRET-signal , suggestive for CD95/CD95-oligomerization .
	manualset3
232897	10	421711	7	NULL	NULL	0	NULL	intracellular FRET-signal	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescence resonance energy transfer ( FRET ) - analysis in Huh7 hepatoma cells , which were cotransfected with CD95-YFP/CD95-CFP revealed that stimulation of these cells with CD95 ligand , proapoptotic bile acids or hyperosmolarity resulted within 30 min in an intracellular FRET-signal , suggestive for CD95/CD95-oligomerization .
	manualset3
232898	11	421711	7	NULL	NULL	0	NULL	CD95/CD95-oligomerization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fluorescence resonance energy transfer ( FRET ) - analysis in Huh7 hepatoma cells , which were cotransfected with CD95-YFP/CD95-CFP revealed that stimulation of these cells with CD95 ligand , proapoptotic bile acids or hyperosmolarity resulted within 30 min in an intracellular FRET-signal , suggestive for CD95/CD95-oligomerization .
	manualset3
232899	1	421712	7	NULL	NULL	0	NULL	 coffee drinking	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We postulate that coffee drinking may have an acute detrimental effect in triggering coronary events and increasing infarct size in selected patient groups , rather than promoting the development of atherosclerosis in the general population , and we propose an alternative approach to explore such an effect in epidemiological studies .
	manualset3
232900	2	421712	7	NULL	NULL	0	NULL	acute detrimental effect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We postulate that coffee drinking may have an acute detrimental effect in triggering coronary events and increasing infarct size in selected patient groups , rather than promoting the development of atherosclerosis in the general population , and we propose an alternative approach to explore such an effect in epidemiological studies .
	manualset3
232901	3	421712	7	NULL	NULL	0	NULL	coronary events	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We postulate that coffee drinking may have an acute detrimental effect in triggering coronary events and increasing infarct size in selected patient groups , rather than promoting the development of atherosclerosis in the general population , and we propose an alternative approach to explore such an effect in epidemiological studies .
	manualset3
232902	4	421712	7	NULL	NULL	0	NULL	 infarct size	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We postulate that coffee drinking may have an acute detrimental effect in triggering coronary events and increasing infarct size in selected patient groups , rather than promoting the development of atherosclerosis in the general population , and we propose an alternative approach to explore such an effect in epidemiological studies .
	manualset3
232903	5	421712	7	NULL	NULL	0	NULL	patient groups 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We postulate that coffee drinking may have an acute detrimental effect in triggering coronary events and increasing infarct size in selected patient groups , rather than promoting the development of atherosclerosis in the general population , and we propose an alternative approach to explore such an effect in epidemiological studies .
	manualset3
232904	6	421712	7	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We postulate that coffee drinking may have an acute detrimental effect in triggering coronary events and increasing infarct size in selected patient groups , rather than promoting the development of atherosclerosis in the general population , and we propose an alternative approach to explore such an effect in epidemiological studies .
	manualset3
232905	7	421712	7	NULL	NULL	NULL	NULL	atherosclerosis 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We postulate that coffee drinking may have an acute detrimental effect in triggering coronary events and increasing infarct size in selected patient groups , rather than promoting the development of atherosclerosis in the general population , and we propose an alternative approach to explore such an effect in epidemiological studies .
	manualset3
232906	8	421712	7	NULL	NULL	0	NULL	general population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We postulate that coffee drinking may have an acute detrimental effect in triggering coronary events and increasing infarct size in selected patient groups , rather than promoting the development of atherosclerosis in the general population , and we propose an alternative approach to explore such an effect in epidemiological studies .
	manualset3
232907	9	421712	7	NULL	NULL	0	NULL	alternative approach	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We postulate that coffee drinking may have an acute detrimental effect in triggering coronary events and increasing infarct size in selected patient groups , rather than promoting the development of atherosclerosis in the general population , and we propose an alternative approach to explore such an effect in epidemiological studies .
	manualset3
232908	10	421712	7	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We postulate that coffee drinking may have an acute detrimental effect in triggering coronary events and increasing infarct size in selected patient groups , rather than promoting the development of atherosclerosis in the general population , and we propose an alternative approach to explore such an effect in epidemiological studies .
	manualset3
232909	11	421712	7	NULL	NULL	0	NULL	epidemiological studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We postulate that coffee drinking may have an acute detrimental effect in triggering coronary events and increasing infarct size in selected patient groups , rather than promoting the development of atherosclerosis in the general population , and we propose an alternative approach to explore such an effect in epidemiological studies .
	manualset3
232910	1	421713	7	NULL	NULL	0	NULL	Nongrowing Escherichia coli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Nongrowing Escherichia coli deprived of an essential amino acid continued to produce peptidoglycan at a rate approximately 30 % of that of growing cells .
	manualset3
232911	2	421713	7	NULL	NULL	0	NULL	 essential amino acid	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Nongrowing Escherichia coli deprived of an essential amino acid continued to produce peptidoglycan at a rate approximately 30 % of that of growing cells .
	manualset3
232912	3	421713	7	NULL	NULL	0	NULL	 peptidoglycan	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Nongrowing Escherichia coli deprived of an essential amino acid continued to produce peptidoglycan at a rate approximately 30 % of that of growing cells .
	manualset3
232913	4	421713	7	NULL	NULL	0	NULL	rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nongrowing Escherichia coli deprived of an essential amino acid continued to produce peptidoglycan at a rate approximately 30 % of that of growing cells .
	manualset3
232914	5	421713	7	NULL	NULL	0	NULL	30 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Nongrowing Escherichia coli deprived of an essential amino acid continued to produce peptidoglycan at a rate approximately 30 % of that of growing cells .
	manualset3
232915	6	421713	7	NULL	NULL	0	NULL	 growing cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Nongrowing Escherichia coli deprived of an essential amino acid continued to produce peptidoglycan at a rate approximately 30 % of that of growing cells .
	manualset3
232916	1	421714	7	NULL	NULL	0	NULL	influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of a chronic vitamin A deficiency on the rat cochlea .
	manualset3
232917	2	421714	7	NULL	NULL	0	NULL	chronic vitamin A deficiency 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of a chronic vitamin A deficiency on the rat cochlea .
	manualset3
232918	3	421714	7	NULL	NULL	0	NULL	rat cochlea	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The influence of a chronic vitamin A deficiency on the rat cochlea .
	manualset3
232919	1	421715	7	NULL	NULL	0	NULL	approach	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An approach to the routine estimation of circulating carcinoembryonic antigen immune complexes in patients with carcinomata of the gastrointestinal tract .
	manualset3
232920	2	421715	7	NULL	NULL	0	NULL	 routine estimation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An approach to the routine estimation of circulating carcinoembryonic antigen immune complexes in patients with carcinomata of the gastrointestinal tract .
	manualset3
232921	3	421715	7	NULL	NULL	0	NULL	circulating carcinoembryonic antigen immune complexes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	An approach to the routine estimation of circulating carcinoembryonic antigen immune complexes in patients with carcinomata of the gastrointestinal tract .
	manualset3
232922	4	421715	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	An approach to the routine estimation of circulating carcinoembryonic antigen immune complexes in patients with carcinomata of the gastrointestinal tract .
	manualset3
232923	5	421715	7	NULL	NULL	0	NULL	carcinomata	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	An approach to the routine estimation of circulating carcinoembryonic antigen immune complexes in patients with carcinomata of the gastrointestinal tract .
	manualset3
232924	6	421715	7	NULL	NULL	0	NULL	gastrointestinal tract 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An approach to the routine estimation of circulating carcinoembryonic antigen immune complexes in patients with carcinomata of the gastrointestinal tract .
	manualset3
232925	1	421716	7	NULL	NULL	0	NULL	Reaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Reaction to skin homografts in thymectomized rats ) .
	manualset3
232926	2	421716	7	NULL	NULL	0	NULL	skin homografts 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Reaction to skin homografts in thymectomized rats ) .
	manualset3
232927	3	421716	7	NULL	NULL	0	NULL	thymectomized rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Reaction to skin homografts in thymectomized rats ) .
	manualset3
232928	1	421717	7	NULL	NULL	0	NULL	proportions  	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportions of EMA-positive sera positive by other assays for CD were 92 % for transglutaminase IgA ( TG-IgA ) , 80 % for gliadin IgA , 84 % for gliadin IgG , 60 % for endomysial IgG ( EMG ) , and 32 % for transglutaminase IgG ( TG-IgG ) .
	manualset3
232929	2	421717	7	NULL	NULL	0	NULL	EMA-positive sera positive	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportions of EMA-positive sera positive by other assays for CD were 92 % for transglutaminase IgA ( TG-IgA ) , 80 % for gliadin IgA , 84 % for gliadin IgG , 60 % for endomysial IgG ( EMG ) , and 32 % for transglutaminase IgG ( TG-IgG ) .
	manualset3
232930	3	421717	7	NULL	NULL	0	NULL	 assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportions of EMA-positive sera positive by other assays for CD were 92 % for transglutaminase IgA ( TG-IgA ) , 80 % for gliadin IgA , 84 % for gliadin IgG , 60 % for endomysial IgG ( EMG ) , and 32 % for transglutaminase IgG ( TG-IgG ) .
	manualset3
232931	4	421717	7	NULL	NULL	0	NULL	CD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportions of EMA-positive sera positive by other assays for CD were 92 % for transglutaminase IgA ( TG-IgA ) , 80 % for gliadin IgA , 84 % for gliadin IgG , 60 % for endomysial IgG ( EMG ) , and 32 % for transglutaminase IgG ( TG-IgG ) .
	manualset3
232932	5	421717	7	NULL	NULL	0	NULL	 92 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportions of EMA-positive sera positive by other assays for CD were 92 % for transglutaminase IgA ( TG-IgA ) , 80 % for gliadin IgA , 84 % for gliadin IgG , 60 % for endomysial IgG ( EMG ) , and 32 % for transglutaminase IgG ( TG-IgG ) .
	manualset3
232933	6	421717	7	NULL	NULL	0	NULL	 transglutaminase IgA ( TG-IgA ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportions of EMA-positive sera positive by other assays for CD were 92 % for transglutaminase IgA ( TG-IgA ) , 80 % for gliadin IgA , 84 % for gliadin IgG , 60 % for endomysial IgG ( EMG ) , and 32 % for transglutaminase IgG ( TG-IgG ) .
	manualset3
232934	7	421717	7	NULL	NULL	0	NULL	80 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportions of EMA-positive sera positive by other assays for CD were 92 % for transglutaminase IgA ( TG-IgA ) , 80 % for gliadin IgA , 84 % for gliadin IgG , 60 % for endomysial IgG ( EMG ) , and 32 % for transglutaminase IgG ( TG-IgG ) .
	manualset3
232935	8	421717	7	NULL	NULL	0	NULL	gliadin IgA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportions of EMA-positive sera positive by other assays for CD were 92 % for transglutaminase IgA ( TG-IgA ) , 80 % for gliadin IgA , 84 % for gliadin IgG , 60 % for endomysial IgG ( EMG ) , and 32 % for transglutaminase IgG ( TG-IgG ) .
	manualset3
232936	9	421717	7	NULL	NULL	0	NULL	84 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportions of EMA-positive sera positive by other assays for CD were 92 % for transglutaminase IgA ( TG-IgA ) , 80 % for gliadin IgA , 84 % for gliadin IgG , 60 % for endomysial IgG ( EMG ) , and 32 % for transglutaminase IgG ( TG-IgG ) .
	manualset3
232937	10	421717	7	NULL	NULL	0	NULL	gliadin IgG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportions of EMA-positive sera positive by other assays for CD were 92 % for transglutaminase IgA ( TG-IgA ) , 80 % for gliadin IgA , 84 % for gliadin IgG , 60 % for endomysial IgG ( EMG ) , and 32 % for transglutaminase IgG ( TG-IgG ) .
	manualset3
232938	11	421717	7	NULL	NULL	0	NULL	60 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportions of EMA-positive sera positive by other assays for CD were 92 % for transglutaminase IgA ( TG-IgA ) , 80 % for gliadin IgA , 84 % for gliadin IgG , 60 % for endomysial IgG ( EMG ) , and 32 % for transglutaminase IgG ( TG-IgG ) .
	manualset3
232939	12	421717	7	NULL	NULL	0	NULL	endomysial IgG ( EMG ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportions of EMA-positive sera positive by other assays for CD were 92 % for transglutaminase IgA ( TG-IgA ) , 80 % for gliadin IgA , 84 % for gliadin IgG , 60 % for endomysial IgG ( EMG ) , and 32 % for transglutaminase IgG ( TG-IgG ) .
	manualset3
232940	13	421717	7	NULL	NULL	0	NULL	32 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportions of EMA-positive sera positive by other assays for CD were 92 % for transglutaminase IgA ( TG-IgA ) , 80 % for gliadin IgA , 84 % for gliadin IgG , 60 % for endomysial IgG ( EMG ) , and 32 % for transglutaminase IgG ( TG-IgG ) .
	manualset3
232941	14	421717	7	NULL	NULL	0	NULL	transglutaminase IgG ( TG-IgG )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The proportions of EMA-positive sera positive by other assays for CD were 92 % for transglutaminase IgA ( TG-IgA ) , 80 % for gliadin IgA , 84 % for gliadin IgG , 60 % for endomysial IgG ( EMG ) , and 32 % for transglutaminase IgG ( TG-IgG ) .
	manualset3
232942	1	421718	7	NULL	NULL	0	NULL	Two photoproducts	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two photoproducts , namely C1 and C2 , purified and characterized by mass spectroscopy and nuclear magnetic resonance ( NMR ) analysis , effectively induced apoptosis in HL60 and M14 cells .
	manualset3
232943	2	421718	7	NULL	NULL	0	NULL	C1 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two photoproducts , namely C1 and C2 , purified and characterized by mass spectroscopy and nuclear magnetic resonance ( NMR ) analysis , effectively induced apoptosis in HL60 and M14 cells .
	manualset3
232944	3	421718	7	NULL	NULL	0	NULL	C2	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two photoproducts , namely C1 and C2 , purified and characterized by mass spectroscopy and nuclear magnetic resonance ( NMR ) analysis , effectively induced apoptosis in HL60 and M14 cells .
	manualset3
232945	4	421718	7	NULL	NULL	0	NULL	mass spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two photoproducts , namely C1 and C2 , purified and characterized by mass spectroscopy and nuclear magnetic resonance ( NMR ) analysis , effectively induced apoptosis in HL60 and M14 cells .
	manualset3
232946	5	421718	7	NULL	NULL	0	NULL	nuclear magnetic resonance ( NMR ) analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two photoproducts , namely C1 and C2 , purified and characterized by mass spectroscopy and nuclear magnetic resonance ( NMR ) analysis , effectively induced apoptosis in HL60 and M14 cells .
	manualset3
232947	6	421718	7	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two photoproducts , namely C1 and C2 , purified and characterized by mass spectroscopy and nuclear magnetic resonance ( NMR ) analysis , effectively induced apoptosis in HL60 and M14 cells .
	manualset3
232948	7	421718	7	NULL	NULL	0	NULL	HL60 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Two photoproducts , namely C1 and C2 , purified and characterized by mass spectroscopy and nuclear magnetic resonance ( NMR ) analysis , effectively induced apoptosis in HL60 and M14 cells .
	manualset3
232949	8	421718	7	NULL	NULL	0	NULL	M14 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Two photoproducts , namely C1 and C2 , purified and characterized by mass spectroscopy and nuclear magnetic resonance ( NMR ) analysis , effectively induced apoptosis in HL60 and M14 cells .
	manualset3
232950	1	421719	7	NULL	NULL	0	NULL	Geobacter sulfurreducens 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Geobacter sulfurreducens is one of a family of microorganisms that oxidize organic compounds , with Fe ( III ) oxide as the terminal electron acceptor .
	manualset3
232951	2	421719	7	NULL	NULL	0	NULL	one 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Geobacter sulfurreducens is one of a family of microorganisms that oxidize organic compounds , with Fe ( III ) oxide as the terminal electron acceptor .
	manualset3
232952	3	421719	7	NULL	NULL	0	NULL	 family	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Geobacter sulfurreducens is one of a family of microorganisms that oxidize organic compounds , with Fe ( III ) oxide as the terminal electron acceptor .
	manualset3
232953	4	421719	7	NULL	NULL	0	NULL	microorganisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Geobacter sulfurreducens is one of a family of microorganisms that oxidize organic compounds , with Fe ( III ) oxide as the terminal electron acceptor .
	manualset3
232954	5	421719	7	NULL	NULL	0	NULL	organic compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Geobacter sulfurreducens is one of a family of microorganisms that oxidize organic compounds , with Fe ( III ) oxide as the terminal electron acceptor .
	manualset3
232955	6	421719	7	NULL	NULL	0	NULL	Fe ( III ) oxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Geobacter sulfurreducens is one of a family of microorganisms that oxidize organic compounds , with Fe ( III ) oxide as the terminal electron acceptor .
	manualset3
232956	7	421719	7	NULL	NULL	0	NULL	terminal electron acceptor 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Geobacter sulfurreducens is one of a family of microorganisms that oxidize organic compounds , with Fe ( III ) oxide as the terminal electron acceptor .
	manualset3
232957	1	421720	7	NULL	NULL	0	NULL	caution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although caution about generalization of the effects to the typical clinical situation is emphasized , the study provides preliminary evidence of a therapeutic benefit from hydration treatments in patients with nodules or polyps .
	manualset3
232958	2	421720	7	NULL	NULL	0	NULL	generalization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although caution about generalization of the effects to the typical clinical situation is emphasized , the study provides preliminary evidence of a therapeutic benefit from hydration treatments in patients with nodules or polyps .
	manualset3
232959	3	421720	7	NULL	NULL	0	NULL	 effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although caution about generalization of the effects to the typical clinical situation is emphasized , the study provides preliminary evidence of a therapeutic benefit from hydration treatments in patients with nodules or polyps .
	manualset3
232960	4	421720	7	NULL	NULL	0	NULL	 clinical situation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although caution about generalization of the effects to the typical clinical situation is emphasized , the study provides preliminary evidence of a therapeutic benefit from hydration treatments in patients with nodules or polyps .
	manualset3
232961	5	421720	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although caution about generalization of the effects to the typical clinical situation is emphasized , the study provides preliminary evidence of a therapeutic benefit from hydration treatments in patients with nodules or polyps .
	manualset3
232962	6	421720	7	NULL	NULL	0	NULL	preliminary evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although caution about generalization of the effects to the typical clinical situation is emphasized , the study provides preliminary evidence of a therapeutic benefit from hydration treatments in patients with nodules or polyps .
	manualset3
232964	7	421720	7	NULL	NULL	0	NULL	therapeutic benefit	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although caution about generalization of the effects to the typical clinical situation is emphasized , the study provides preliminary evidence of a therapeutic benefit from hydration treatments in patients with nodules or polyps .
	manualset3
232965	8	421720	7	NULL	NULL	0	NULL	hydration treatments 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although caution about generalization of the effects to the typical clinical situation is emphasized , the study provides preliminary evidence of a therapeutic benefit from hydration treatments in patients with nodules or polyps .
	manualset3
232966	9	421720	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although caution about generalization of the effects to the typical clinical situation is emphasized , the study provides preliminary evidence of a therapeutic benefit from hydration treatments in patients with nodules or polyps .
	manualset3
232967	10	421720	7	NULL	NULL	0	NULL	 nodules	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although caution about generalization of the effects to the typical clinical situation is emphasized , the study provides preliminary evidence of a therapeutic benefit from hydration treatments in patients with nodules or polyps .
	manualset3
232968	11	421720	7	NULL	NULL	0	NULL	polyps	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although caution about generalization of the effects to the typical clinical situation is emphasized , the study provides preliminary evidence of a therapeutic benefit from hydration treatments in patients with nodules or polyps .
	manualset3
232969	1	421721	7	NULL	NULL	0	NULL	results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of monitoring of the aerosol from traffic , dust storms and forest fires in 30-km zone of the Chernobyl nuclear power plant and other regions are compared .
	manualset3
232970	2	421721	7	NULL	NULL	0	NULL	monitoring	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of monitoring of the aerosol from traffic , dust storms and forest fires in 30-km zone of the Chernobyl nuclear power plant and other regions are compared .
	manualset3
232971	3	421721	7	NULL	NULL	0	NULL	aerosol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of monitoring of the aerosol from traffic , dust storms and forest fires in 30-km zone of the Chernobyl nuclear power plant and other regions are compared .
	manualset3
232972	4	421721	7	NULL	NULL	0	NULL	 traffic	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of monitoring of the aerosol from traffic , dust storms and forest fires in 30-km zone of the Chernobyl nuclear power plant and other regions are compared .
	manualset3
232973	5	421721	7	NULL	NULL	0	NULL	dust storms 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of monitoring of the aerosol from traffic , dust storms and forest fires in 30-km zone of the Chernobyl nuclear power plant and other regions are compared .
	manualset3
232974	6	421721	7	NULL	NULL	0	NULL	 forest fires	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of monitoring of the aerosol from traffic , dust storms and forest fires in 30-km zone of the Chernobyl nuclear power plant and other regions are compared .
	manualset3
232975	7	421721	7	NULL	NULL	NULL	NULL	30-km zone	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of monitoring of the aerosol from traffic , dust storms and forest fires in 30-km zone of the Chernobyl nuclear power plant and other regions are compared .
	manualset3
232976	8	421721	7	NULL	NULL	0	NULL	 Chernobyl nuclear power plant 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The results of monitoring of the aerosol from traffic , dust storms and forest fires in 30-km zone of the Chernobyl nuclear power plant and other regions are compared .
	manualset3
232977	9	421721	7	NULL	NULL	NULL	NULL	 regions	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The results of monitoring of the aerosol from traffic , dust storms and forest fires in 30-km zone of the Chernobyl nuclear power plant and other regions are compared .
	manualset3
232978	1	421722	7	NULL	NULL	0	NULL	selective capture	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The selective capture of Cs ( + ) from solution is relevant to the remediation of nuclear waste and remains a significant challenge .
	manualset3
232979	2	421722	7	NULL	NULL	0	NULL	Cs ( + )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The selective capture of Cs ( + ) from solution is relevant to the remediation of nuclear waste and remains a significant challenge .
	manualset3
232980	3	421722	7	NULL	NULL	0	NULL	solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The selective capture of Cs ( + ) from solution is relevant to the remediation of nuclear waste and remains a significant challenge .
	manualset3
232981	4	421722	7	NULL	NULL	0	NULL	remediation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The selective capture of Cs ( + ) from solution is relevant to the remediation of nuclear waste and remains a significant challenge .
	manualset3
232982	5	421722	7	NULL	NULL	0	NULL	nuclear waste	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The selective capture of Cs ( + ) from solution is relevant to the remediation of nuclear waste and remains a significant challenge .
	manualset3
232983	6	421722	7	NULL	NULL	0	NULL	challenge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The selective capture of Cs ( + ) from solution is relevant to the remediation of nuclear waste and remains a significant challenge .
	manualset3
232984	1	421723	7	NULL	NULL	0	NULL	Confocal laser scanning microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Confocal laser scanning microscopy indicated nuclear and nucleolar accumulation of fluoresceinated granzyme B by isolated nuclei .
	manualset3
232986	2	421723	7	NULL	NULL	0	NULL	 nuclear accumulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Confocal laser scanning microscopy indicated nuclear and nucleolar accumulation of fluoresceinated granzyme B by isolated nuclei .
	manualset3
232987	3	421723	7	NULL	NULL	0	NULL	nucleolar accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Confocal laser scanning microscopy indicated nuclear and nucleolar accumulation of fluoresceinated granzyme B by isolated nuclei .
	manualset3
232988	4	421723	7	NULL	NULL	0	NULL	fluoresceinated granzyme B 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Confocal laser scanning microscopy indicated nuclear and nucleolar accumulation of fluoresceinated granzyme B by isolated nuclei .
	manualset3
232989	5	421723	7	NULL	NULL	0	NULL	 isolated nuclei	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Confocal laser scanning microscopy indicated nuclear and nucleolar accumulation of fluoresceinated granzyme B by isolated nuclei .
	manualset3
232990	1	421724	7	NULL	NULL	0	NULL	 indication 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There was some indication of increased concentration of C-reactive protein ( CRP ) and no difference in haptoglobin levels .
	manualset3
232991	2	421724	7	NULL	NULL	0	NULL	increased concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was some indication of increased concentration of C-reactive protein ( CRP ) and no difference in haptoglobin levels .
	manualset3
232992	3	421724	7	NULL	NULL	0	NULL	C-reactive protein ( CRP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	There was some indication of increased concentration of C-reactive protein ( CRP ) and no difference in haptoglobin levels .
	manualset3
232993	4	421724	7	NULL	NULL	0	NULL	no difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	There was some indication of increased concentration of C-reactive protein ( CRP ) and no difference in haptoglobin levels .
	manualset3
232994	5	421724	7	NULL	NULL	0	NULL	haptoglobin levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was some indication of increased concentration of C-reactive protein ( CRP ) and no difference in haptoglobin levels .
	manualset3
232995	1	421725	7	NULL	NULL	0	NULL	17 unique proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 17 unique proteins that were identified , five have often been cited as tumor biomarkers .
	manualset3
232996	2	421725	7	NULL	NULL	0	NULL	five	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 17 unique proteins that were identified , five have often been cited as tumor biomarkers .
	manualset3
232997	3	421725	7	NULL	NULL	0	NULL	tumor biomarkers	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Of the 17 unique proteins that were identified , five have often been cited as tumor biomarkers .
	manualset3
232998	1	421726	7	NULL	NULL	0	NULL	changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Changes in cerebral blood flow , cerebral metabolites , and breathing movements in the sheep fetus following asphyxia produced by occlusion of the umbilical cord .
	manualset3
232999	2	421726	7	NULL	NULL	0	NULL	cerebral blood flow	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Changes in cerebral blood flow , cerebral metabolites , and breathing movements in the sheep fetus following asphyxia produced by occlusion of the umbilical cord .
	manualset3
233000	3	421726	7	NULL	NULL	0	NULL	cerebral metabolites	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Changes in cerebral blood flow , cerebral metabolites , and breathing movements in the sheep fetus following asphyxia produced by occlusion of the umbilical cord .
	manualset3
233001	4	421726	7	NULL	NULL	0	NULL	 breathing movements	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Changes in cerebral blood flow , cerebral metabolites , and breathing movements in the sheep fetus following asphyxia produced by occlusion of the umbilical cord .
	manualset3
233002	5	421726	7	NULL	NULL	0	NULL	sheep fetus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Changes in cerebral blood flow , cerebral metabolites , and breathing movements in the sheep fetus following asphyxia produced by occlusion of the umbilical cord .
	manualset3
233003	6	421726	7	NULL	NULL	0	NULL	 asphyxia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Changes in cerebral blood flow , cerebral metabolites , and breathing movements in the sheep fetus following asphyxia produced by occlusion of the umbilical cord .
	manualset3
233004	7	421726	7	NULL	NULL	NULL	NULL	occlusion	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Changes in cerebral blood flow , cerebral metabolites , and breathing movements in the sheep fetus following asphyxia produced by occlusion of the umbilical cord .
	manualset3
233005	8	421726	7	NULL	NULL	0	NULL	umbilical cord 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Changes in cerebral blood flow , cerebral metabolites , and breathing movements in the sheep fetus following asphyxia produced by occlusion of the umbilical cord .
	manualset3
233006	1	421727	7	NULL	NULL	0	NULL	 woman 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The woman preferred a system with a contact microphone since this was virtually unaffected by environmental noise .
	manualset3
233007	2	421727	7	NULL	NULL	0	NULL	system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The woman preferred a system with a contact microphone since this was virtually unaffected by environmental noise .
	manualset3
233008	3	421727	7	NULL	NULL	0	NULL	contact microphone	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The woman preferred a system with a contact microphone since this was virtually unaffected by environmental noise .
	manualset3
233009	4	421727	7	NULL	NULL	NULL	NULL	environmental noise	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The woman preferred a system with a contact microphone since this was virtually unaffected by environmental noise .
	manualset3
233010	1	421728	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There is little clear evidence about the most effective way that the subject of racism can be explored in the classroom setting .
	manualset3
233011	2	421728	7	NULL	NULL	0	NULL	effective way 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is little clear evidence about the most effective way that the subject of racism can be explored in the classroom setting .
	manualset3
233012	3	421728	7	NULL	NULL	NULL	NULL	subject	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There is little clear evidence about the most effective way that the subject of racism can be explored in the classroom setting .
	manualset3
233013	4	421728	7	NULL	NULL	NULL	NULL	racism	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There is little clear evidence about the most effective way that the subject of racism can be explored in the classroom setting .
	manualset3
233014	5	421728	7	NULL	NULL	0	NULL	classroom setting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There is little clear evidence about the most effective way that the subject of racism can be explored in the classroom setting .
	manualset3
233015	1	421729	7	NULL	NULL	0	NULL	approximate method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An approximate method for determining the correct path of a beam through the coating is derived and the path is illustrated using a Gaussian incident beam and tracing the position of the peak field of the beam as it traverses the coating .
	manualset3
233016	2	421729	7	NULL	NULL	0	NULL	correct path	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An approximate method for determining the correct path of a beam through the coating is derived and the path is illustrated using a Gaussian incident beam and tracing the position of the peak field of the beam as it traverses the coating .
	manualset3
233017	3	421729	7	NULL	NULL	0	NULL	 beam	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	An approximate method for determining the correct path of a beam through the coating is derived and the path is illustrated using a Gaussian incident beam and tracing the position of the peak field of the beam as it traverses the coating .
	manualset3
233018	4	421729	7	NULL	NULL	0	NULL	coating	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An approximate method for determining the correct path of a beam through the coating is derived and the path is illustrated using a Gaussian incident beam and tracing the position of the peak field of the beam as it traverses the coating .
	manualset3
233019	5	421729	7	NULL	NULL	0	NULL	Gaussian incident beam	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	An approximate method for determining the correct path of a beam through the coating is derived and the path is illustrated using a Gaussian incident beam and tracing the position of the peak field of the beam as it traverses the coating .
	manualset3
233020	6	421729	7	NULL	NULL	0	NULL	tracing 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An approximate method for determining the correct path of a beam through the coating is derived and the path is illustrated using a Gaussian incident beam and tracing the position of the peak field of the beam as it traverses the coating .
	manualset3
233021	7	421729	7	NULL	NULL	0	NULL	position 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An approximate method for determining the correct path of a beam through the coating is derived and the path is illustrated using a Gaussian incident beam and tracing the position of the peak field of the beam as it traverses the coating .
	manualset3
233022	8	421729	7	NULL	NULL	0	NULL	peak field 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	An approximate method for determining the correct path of a beam through the coating is derived and the path is illustrated using a Gaussian incident beam and tracing the position of the peak field of the beam as it traverses the coating .
	manualset3
233023	9	421729	7	NULL	NULL	0	NULL	beam	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	An approximate method for determining the correct path of a beam through the coating is derived and the path is illustrated using a Gaussian incident beam and tracing the position of the peak field of the beam as it traverses the coating .
	manualset3
233024	10	421729	7	NULL	NULL	0	NULL	coating	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An approximate method for determining the correct path of a beam through the coating is derived and the path is illustrated using a Gaussian incident beam and tracing the position of the peak field of the beam as it traverses the coating .
	manualset3
233025	1	421730	7	NULL	NULL	0	NULL	Two cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Two cases of streptococcal endocarditis lenta treated by oral penicillin V ) .
	manualset3
233026	2	421730	7	NULL	NULL	0	NULL	streptococcal endocarditis lenta	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Two cases of streptococcal endocarditis lenta treated by oral penicillin V ) .
	manualset3
233027	3	421730	7	NULL	NULL	0	NULL	oral penicillin V	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Two cases of streptococcal endocarditis lenta treated by oral penicillin V ) .
	manualset3
233268	1	421731	7	NULL	NULL	0	NULL	Hepatitis D virus superinfection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatitis D virus superinfection remains a rare occurrence in non-drug abusers in Hong Kong .
	manualset3
233269	2	421731	7	NULL	NULL	0	NULL	non-drug abusers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatitis D virus superinfection remains a rare occurrence in non-drug abusers in Hong Kong .
	manualset3
233270	3	421731	7	NULL	NULL	0	NULL	Hong Kong	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Hepatitis D virus superinfection remains a rare occurrence in non-drug abusers in Hong Kong .
	manualset3
233271	1	421732	7	NULL	NULL	0	NULL	Liver biopsies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver biopsies performed in these patients revealed histological alterations consistent with toxic liver injury .
	manualset3
233272	2	421732	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver biopsies performed in these patients revealed histological alterations consistent with toxic liver injury .
	manualset3
233273	3	421732	7	NULL	NULL	0	NULL	histological alterations 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver biopsies performed in these patients revealed histological alterations consistent with toxic liver injury .
	manualset3
233274	4	421732	7	NULL	NULL	0	NULL	toxic liver injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver biopsies performed in these patients revealed histological alterations consistent with toxic liver injury .
	manualset3
233275	1	421733	7	NULL	NULL	0	NULL	penultimate step 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The penultimate step in carnitine biosynthesis is mediated by gamma-trimethylaminobutyraldehyde dehydrogenase ( EC 1.2.1.47 ) , a cytosolic NAD ( + ) - dependent aldehyde dehydrogenase that converts gamma-trimethylaminobutyraldehyde into gamma-butyrobetaine .
	manualset3
233276	2	421733	7	NULL	NULL	0	NULL	carnitine biosynthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The penultimate step in carnitine biosynthesis is mediated by gamma-trimethylaminobutyraldehyde dehydrogenase ( EC 1.2.1.47 ) , a cytosolic NAD ( + ) - dependent aldehyde dehydrogenase that converts gamma-trimethylaminobutyraldehyde into gamma-butyrobetaine .
	manualset3
233277	3	421733	7	NULL	NULL	0	NULL	gamma-trimethylaminobutyraldehyde dehydrogenase ( EC 1.2.1.47 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The penultimate step in carnitine biosynthesis is mediated by gamma-trimethylaminobutyraldehyde dehydrogenase ( EC 1.2.1.47 ) , a cytosolic NAD ( + ) - dependent aldehyde dehydrogenase that converts gamma-trimethylaminobutyraldehyde into gamma-butyrobetaine .
	manualset3
233278	4	421733	7	NULL	NULL	0	NULL	cytosolic NAD ( + ) - dependent aldehyde dehydrogenase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The penultimate step in carnitine biosynthesis is mediated by gamma-trimethylaminobutyraldehyde dehydrogenase ( EC 1.2.1.47 ) , a cytosolic NAD ( + ) - dependent aldehyde dehydrogenase that converts gamma-trimethylaminobutyraldehyde into gamma-butyrobetaine .
	manualset3
233279	5	421733	7	NULL	NULL	0	NULL	gamma-trimethylaminobutyraldehyde	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The penultimate step in carnitine biosynthesis is mediated by gamma-trimethylaminobutyraldehyde dehydrogenase ( EC 1.2.1.47 ) , a cytosolic NAD ( + ) - dependent aldehyde dehydrogenase that converts gamma-trimethylaminobutyraldehyde into gamma-butyrobetaine .
	manualset3
233280	6	421733	7	NULL	NULL	0	NULL	gamma-butyrobetaine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The penultimate step in carnitine biosynthesis is mediated by gamma-trimethylaminobutyraldehyde dehydrogenase ( EC 1.2.1.47 ) , a cytosolic NAD ( + ) - dependent aldehyde dehydrogenase that converts gamma-trimethylaminobutyraldehyde into gamma-butyrobetaine .
	manualset3
233281	1	421734	7	NULL	NULL	0	NULL	summary	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , it was diagnosed that the patient had synchronous double primary lung adenocarcinomas of T1 N0 M0 pathological stage and 12 solitary atypical adenomatous hyperplasias .
	manualset3
233282	2	421734	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , it was diagnosed that the patient had synchronous double primary lung adenocarcinomas of T1 N0 M0 pathological stage and 12 solitary atypical adenomatous hyperplasias .
	manualset3
233283	3	421734	7	NULL	NULL	0	NULL	double primary lung adenocarcinomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , it was diagnosed that the patient had synchronous double primary lung adenocarcinomas of T1 N0 M0 pathological stage and 12 solitary atypical adenomatous hyperplasias .
	manualset3
233284	4	421734	7	NULL	NULL	0	NULL	T1 N0 M0 pathological stage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , it was diagnosed that the patient had synchronous double primary lung adenocarcinomas of T1 N0 M0 pathological stage and 12 solitary atypical adenomatous hyperplasias .
	manualset3
233285	5	421734	7	NULL	NULL	0	NULL	12 solitary atypical adenomatous hyperplasias 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , it was diagnosed that the patient had synchronous double primary lung adenocarcinomas of T1 N0 M0 pathological stage and 12 solitary atypical adenomatous hyperplasias .
	manualset3
233286	1	421735	7	NULL	NULL	0	NULL	Mishandling 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mishandling of Ca ( 2 + ) is a central cause of both contractile dysfunction and arrhythmias in pathophysiological conditions such as heart failure ( HF ) .
	manualset3
233287	2	421735	7	NULL	NULL	0	NULL	Ca ( 2 + )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Mishandling of Ca ( 2 + ) is a central cause of both contractile dysfunction and arrhythmias in pathophysiological conditions such as heart failure ( HF ) .
	manualset3
233288	3	421735	7	NULL	NULL	0	NULL	central cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mishandling of Ca ( 2 + ) is a central cause of both contractile dysfunction and arrhythmias in pathophysiological conditions such as heart failure ( HF ) .
	manualset3
233289	4	421735	7	NULL	NULL	0	NULL	contractile dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mishandling of Ca ( 2 + ) is a central cause of both contractile dysfunction and arrhythmias in pathophysiological conditions such as heart failure ( HF ) .
	manualset3
233290	5	421735	7	NULL	NULL	0	NULL	arrhythmias	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mishandling of Ca ( 2 + ) is a central cause of both contractile dysfunction and arrhythmias in pathophysiological conditions such as heart failure ( HF ) .
	manualset3
233291	6	421735	7	NULL	NULL	0	NULL	pathophysiological conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mishandling of Ca ( 2 + ) is a central cause of both contractile dysfunction and arrhythmias in pathophysiological conditions such as heart failure ( HF ) .
	manualset3
233292	7	421735	7	NULL	NULL	0	NULL	heart failure ( HF )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Mishandling of Ca ( 2 + ) is a central cause of both contractile dysfunction and arrhythmias in pathophysiological conditions such as heart failure ( HF ) .
	manualset3
233293	1	421736	7	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that 5-aza-dCyd is more effective than ara-C against the ic L1210 leukemia .
	manualset3
233294	2	421736	7	NULL	NULL	0	NULL	5-aza-dCyd 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that 5-aza-dCyd is more effective than ara-C against the ic L1210 leukemia .
	manualset3
233295	3	421736	7	NULL	NULL	0	NULL	ara-C	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that 5-aza-dCyd is more effective than ara-C against the ic L1210 leukemia .
	manualset3
233296	4	421736	7	NULL	NULL	0	NULL	L1210 leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that 5-aza-dCyd is more effective than ara-C against the ic L1210 leukemia .
	manualset3
233297	1	421737	7	NULL	NULL	0	NULL	Heptane	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Heptane showed greater TEWL values and erythema score than other two chemicals ( xylene and hexadecane ) .
	manualset3
233298	2	421737	7	NULL	NULL	0	NULL	TEWL values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Heptane showed greater TEWL values and erythema score than other two chemicals ( xylene and hexadecane ) .
	manualset3
233299	3	421737	7	NULL	NULL	0	NULL	erythema score	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Heptane showed greater TEWL values and erythema score than other two chemicals ( xylene and hexadecane ) .
	manualset3
233300	4	421737	7	NULL	NULL	0	NULL	two chemicals 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Heptane showed greater TEWL values and erythema score than other two chemicals ( xylene and hexadecane ) .
	manualset3
233301	5	421737	7	NULL	NULL	0	NULL	xylene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Heptane showed greater TEWL values and erythema score than other two chemicals ( xylene and hexadecane ) .
	manualset3
233302	6	421737	7	NULL	NULL	0	NULL	hexadecane	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Heptane showed greater TEWL values and erythema score than other two chemicals ( xylene and hexadecane ) .
	manualset3
233398	1	421738	7	NULL	NULL	0	NULL	approximation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An approximation of the free cholesterol , triglycerides , and individual cholesteryl esters is obtained from single chromatograms of isopropanol extracts of serum if the first mobile phase is used .
	manualset3
233399	2	421738	7	NULL	NULL	0	NULL	free cholesterol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An approximation of the free cholesterol , triglycerides , and individual cholesteryl esters is obtained from single chromatograms of isopropanol extracts of serum if the first mobile phase is used .
	manualset3
233401	3	421738	7	NULL	NULL	0	NULL	triglycerides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An approximation of the free cholesterol , triglycerides , and individual cholesteryl esters is obtained from single chromatograms of isopropanol extracts of serum if the first mobile phase is used .
	manualset3
233402	4	421738	7	NULL	NULL	0	NULL	cholesteryl esters 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An approximation of the free cholesterol , triglycerides , and individual cholesteryl esters is obtained from single chromatograms of isopropanol extracts of serum if the first mobile phase is used .
	manualset3
233403	5	421738	7	NULL	NULL	0	NULL	single chromatograms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An approximation of the free cholesterol , triglycerides , and individual cholesteryl esters is obtained from single chromatograms of isopropanol extracts of serum if the first mobile phase is used .
	manualset3
233404	6	421738	7	NULL	NULL	0	NULL	 isopropanol extracts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An approximation of the free cholesterol , triglycerides , and individual cholesteryl esters is obtained from single chromatograms of isopropanol extracts of serum if the first mobile phase is used .
	manualset3
233405	7	421738	7	NULL	NULL	0	NULL	serum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An approximation of the free cholesterol , triglycerides , and individual cholesteryl esters is obtained from single chromatograms of isopropanol extracts of serum if the first mobile phase is used .
	manualset3
233406	8	421738	7	NULL	NULL	0	NULL	 first mobile phase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An approximation of the free cholesterol , triglycerides , and individual cholesteryl esters is obtained from single chromatograms of isopropanol extracts of serum if the first mobile phase is used .
	manualset3
233421	1	421739	7	NULL	NULL	0	NULL	crystallographic structures	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the crystallographic structures of the human pancreatic lipase and of a human lipase-porcine colipase complex have been solved , no refined structure of pancreatic lipase has yet been published .
	manualset3
233422	2	421739	7	NULL	NULL	0	NULL	 human pancreatic lipase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the crystallographic structures of the human pancreatic lipase and of a human lipase-porcine colipase complex have been solved , no refined structure of pancreatic lipase has yet been published .
	manualset3
233423	3	421739	7	NULL	NULL	0	NULL	human lipase-porcine colipase complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the crystallographic structures of the human pancreatic lipase and of a human lipase-porcine colipase complex have been solved , no refined structure of pancreatic lipase has yet been published .
	manualset3
233424	4	421739	7	NULL	NULL	0	NULL	no refined structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the crystallographic structures of the human pancreatic lipase and of a human lipase-porcine colipase complex have been solved , no refined structure of pancreatic lipase has yet been published .
	manualset3
233425	5	421739	7	NULL	NULL	0	NULL	 pancreatic lipase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although the crystallographic structures of the human pancreatic lipase and of a human lipase-porcine colipase complex have been solved , no refined structure of pancreatic lipase has yet been published .
	manualset3
233426	1	421740	7	NULL	NULL	0	NULL	Metal stress	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Metal stress decreased diversity effects on leaf decomposition in assemblages containing the functional type from the unpolluted site , probably due to competitive interactions between fungi .
	manualset3
233427	2	421740	7	NULL	NULL	0	NULL	diversity effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Metal stress decreased diversity effects on leaf decomposition in assemblages containing the functional type from the unpolluted site , probably due to competitive interactions between fungi .
	manualset3
233428	3	421740	7	NULL	NULL	0	NULL	leaf decomposition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Metal stress decreased diversity effects on leaf decomposition in assemblages containing the functional type from the unpolluted site , probably due to competitive interactions between fungi .
	manualset3
233429	4	421740	7	NULL	NULL	0	NULL	assemblages 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Metal stress decreased diversity effects on leaf decomposition in assemblages containing the functional type from the unpolluted site , probably due to competitive interactions between fungi .
	manualset3
233430	5	421740	7	NULL	NULL	NULL	NULL	functional type	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Metal stress decreased diversity effects on leaf decomposition in assemblages containing the functional type from the unpolluted site , probably due to competitive interactions between fungi .
	manualset3
233431	6	421740	7	NULL	NULL	0	NULL	unpolluted site	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Metal stress decreased diversity effects on leaf decomposition in assemblages containing the functional type from the unpolluted site , probably due to competitive interactions between fungi .
	manualset3
233432	7	421740	7	NULL	NULL	0	NULL	competitive interactions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Metal stress decreased diversity effects on leaf decomposition in assemblages containing the functional type from the unpolluted site , probably due to competitive interactions between fungi .
	manualset3
233433	8	421740	7	NULL	NULL	0	NULL	 fungi	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Metal stress decreased diversity effects on leaf decomposition in assemblages containing the functional type from the unpolluted site , probably due to competitive interactions between fungi .
	manualset3
233441	1	421741	7	NULL	NULL	0	NULL	BF4 -	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	BF4 - , the least hydrated and polarizable anion of the set , has one of the largest gammaX - values .
	manualset3
233442	2	421741	7	NULL	NULL	0	NULL	polarizable anion 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	BF4 - , the least hydrated and polarizable anion of the set , has one of the largest gammaX - values .
	manualset3
233443	3	421741	7	NULL	NULL	0	NULL	set	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	BF4 - , the least hydrated and polarizable anion of the set , has one of the largest gammaX - values .
	manualset3
233444	4	421741	7	NULL	NULL	0	NULL	 largest gammaX - values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	BF4 - , the least hydrated and polarizable anion of the set , has one of the largest gammaX - values .
	manualset3
233445	1	421742	7	NULL	NULL	0	NULL	increased mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no increased mortality from lymphatic and hematopoietic cancers overall or from any specific hematological malignancies .
	manualset3
233446	2	421742	7	NULL	NULL	0	NULL	lymphatic cancers	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no increased mortality from lymphatic and hematopoietic cancers overall or from any specific hematological malignancies .
	manualset3
233447	3	421742	7	NULL	NULL	0	NULL	hematopoietic cancers	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no increased mortality from lymphatic and hematopoietic cancers overall or from any specific hematological malignancies .
	manualset3
233448	4	421742	7	NULL	NULL	0	NULL	hematological malignancies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no increased mortality from lymphatic and hematopoietic cancers overall or from any specific hematological malignancies .
	manualset3
233449	1	421743	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The use of telephone for counseling diabetic patients : a descriptive and pedagogic approach ) .
	manualset3
233450	2	421743	7	NULL	NULL	0	NULL	telephone	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	( The use of telephone for counseling diabetic patients : a descriptive and pedagogic approach ) .
	manualset3
233451	3	421743	7	NULL	NULL	0	NULL	diabetic patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( The use of telephone for counseling diabetic patients : a descriptive and pedagogic approach ) .
	manualset3
233452	4	421743	7	NULL	NULL	0	NULL	descriptive approach	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The use of telephone for counseling diabetic patients : a descriptive and pedagogic approach ) .
	manualset3
233453	5	421743	7	NULL	NULL	0	NULL	pedagogic approach	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The use of telephone for counseling diabetic patients : a descriptive and pedagogic approach ) .
	manualset3
233454	1	421744	7	NULL	NULL	NULL	NULL	single-molecule ferritin 	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A single-molecule ferritin picking-up process was realized with the use of AFM , which was enhanced by employing controlled dendron surface chemistry .
	manualset3
233455	2	421744	7	NULL	NULL	0	NULL	picking-up process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A single-molecule ferritin picking-up process was realized with the use of AFM , which was enhanced by employing controlled dendron surface chemistry .
	manualset3
233456	3	421744	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A single-molecule ferritin picking-up process was realized with the use of AFM , which was enhanced by employing controlled dendron surface chemistry .
	manualset3
233457	4	421744	7	NULL	NULL	NULL	NULL	AFM	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A single-molecule ferritin picking-up process was realized with the use of AFM , which was enhanced by employing controlled dendron surface chemistry .
	manualset3
233458	5	421744	7	NULL	NULL	0	NULL	controlled dendron surface chemistry	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A single-molecule ferritin picking-up process was realized with the use of AFM , which was enhanced by employing controlled dendron surface chemistry .
	manualset3
233459	1	421745	7	NULL	NULL	0	NULL	DXR-mAb 9.2.27 immunoconjugates	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Most significantly , DXR-mAb 9.2.27 immunoconjugates specifically suppressed the growth of established tumors in vivo and prolonged the life-span of tumor-bearing nude mice .
	manualset3
233460	2	421745	7	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Most significantly , DXR-mAb 9.2.27 immunoconjugates specifically suppressed the growth of established tumors in vivo and prolonged the life-span of tumor-bearing nude mice .
	manualset3
233461	3	421745	7	NULL	NULL	0	NULL	tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Most significantly , DXR-mAb 9.2.27 immunoconjugates specifically suppressed the growth of established tumors in vivo and prolonged the life-span of tumor-bearing nude mice .
	manualset3
233462	4	421745	7	NULL	NULL	0	NULL	life-span	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Most significantly , DXR-mAb 9.2.27 immunoconjugates specifically suppressed the growth of established tumors in vivo and prolonged the life-span of tumor-bearing nude mice .
	manualset3
233463	5	421745	7	NULL	NULL	0	NULL	tumor-bearing nude mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Most significantly , DXR-mAb 9.2.27 immunoconjugates specifically suppressed the growth of established tumors in vivo and prolonged the life-span of tumor-bearing nude mice .
	manualset3
233464	1	421746	7	NULL	NULL	0	NULL	Functional diagnosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional diagnosis of the affected parts of the respiratory system is helpful in choosing an optimal treatment schedule , promoting improvement of the long-term results of both conservative and surgical treatment of patients with chronic respiratory pathology .
	manualset3
233465	2	421746	7	NULL	NULL	0	NULL	affected parts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional diagnosis of the affected parts of the respiratory system is helpful in choosing an optimal treatment schedule , promoting improvement of the long-term results of both conservative and surgical treatment of patients with chronic respiratory pathology .
	manualset3
233466	3	421746	7	NULL	NULL	0	NULL	respiratory system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional diagnosis of the affected parts of the respiratory system is helpful in choosing an optimal treatment schedule , promoting improvement of the long-term results of both conservative and surgical treatment of patients with chronic respiratory pathology .
	manualset3
233467	4	421746	7	NULL	NULL	0	NULL	optimal treatment schedule	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional diagnosis of the affected parts of the respiratory system is helpful in choosing an optimal treatment schedule , promoting improvement of the long-term results of both conservative and surgical treatment of patients with chronic respiratory pathology .
	manualset3
233468	5	421746	7	NULL	NULL	0	NULL	 improvement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional diagnosis of the affected parts of the respiratory system is helpful in choosing an optimal treatment schedule , promoting improvement of the long-term results of both conservative and surgical treatment of patients with chronic respiratory pathology .
	manualset3
233469	6	421746	7	NULL	NULL	0	NULL	 long-term results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional diagnosis of the affected parts of the respiratory system is helpful in choosing an optimal treatment schedule , promoting improvement of the long-term results of both conservative and surgical treatment of patients with chronic respiratory pathology .
	manualset3
233470	7	421746	7	NULL	NULL	0	NULL	 conservative treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional diagnosis of the affected parts of the respiratory system is helpful in choosing an optimal treatment schedule , promoting improvement of the long-term results of both conservative and surgical treatment of patients with chronic respiratory pathology .
	manualset3
233471	8	421746	7	NULL	NULL	0	NULL	surgical treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional diagnosis of the affected parts of the respiratory system is helpful in choosing an optimal treatment schedule , promoting improvement of the long-term results of both conservative and surgical treatment of patients with chronic respiratory pathology .
	manualset3
233472	9	421746	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional diagnosis of the affected parts of the respiratory system is helpful in choosing an optimal treatment schedule , promoting improvement of the long-term results of both conservative and surgical treatment of patients with chronic respiratory pathology .
	manualset3
233473	10	421746	7	NULL	NULL	0	NULL	chronic respiratory pathology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional diagnosis of the affected parts of the respiratory system is helpful in choosing an optimal treatment schedule , promoting improvement of the long-term results of both conservative and surgical treatment of patients with chronic respiratory pathology .
	manualset3
233474	1	421747	7	NULL	NULL	0	NULL	arbitrary classification scheme	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An arbitrary classification scheme was proposed based on the magnitude of deviation ( d ) as : additive ( & lt ; or = 10 % , class-I ) and moderately ( 10 & lt ; d & lt ; or = 30 % , class-II ) , highly ( 30 & lt ; d & lt ; or = 50 % , class-III ) and very highly ( ) 50 % , class-IV ) antagonistic/synergistic .
	manualset3
233475	2	421747	7	NULL	NULL	0	NULL	magnitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An arbitrary classification scheme was proposed based on the magnitude of deviation ( d ) as : additive ( & lt ; or = 10 % , class-I ) and moderately ( 10 & lt ; d & lt ; or = 30 % , class-II ) , highly ( 30 & lt ; d & lt ; or = 50 % , class-III ) and very highly ( ) 50 % , class-IV ) antagonistic/synergistic .
	manualset3
233476	3	421747	7	NULL	NULL	0	NULL	deviation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An arbitrary classification scheme was proposed based on the magnitude of deviation ( d ) as : additive ( & lt ; or = 10 % , class-I ) and moderately ( 10 & lt ; d & lt ; or = 30 % , class-II ) , highly ( 30 & lt ; d & lt ; or = 50 % , class-III ) and very highly ( ) 50 % , class-IV ) antagonistic/synergistic .
	manualset3
233477	4	421747	7	NULL	NULL	0	NULL	 & lt	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An arbitrary classification scheme was proposed based on the magnitude of deviation ( d ) as : additive ( & lt ; or = 10 % , class-I ) and moderately ( 10 & lt ; d & lt ; or = 30 % , class-II ) , highly ( 30 & lt ; d & lt ; or = 50 % , class-III ) and very highly ( ) 50 % , class-IV ) antagonistic/synergistic .
	manualset3
233478	5	421747	7	NULL	NULL	0	NULL	10 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An arbitrary classification scheme was proposed based on the magnitude of deviation ( d ) as : additive ( & lt ; or = 10 % , class-I ) and moderately ( 10 & lt ; d & lt ; or = 30 % , class-II ) , highly ( 30 & lt ; d & lt ; or = 50 % , class-III ) and very highly ( ) 50 % , class-IV ) antagonistic/synergistic .
	manualset3
233479	6	421747	7	NULL	NULL	NULL	NULL	class-I	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An arbitrary classification scheme was proposed based on the magnitude of deviation ( d ) as : additive ( & lt ; or = 10 % , class-I ) and moderately ( 10 & lt ; d & lt ; or = 30 % , class-II ) , highly ( 30 & lt ; d & lt ; or = 50 % , class-III ) and very highly ( ) 50 % , class-IV ) antagonistic/synergistic .
	manualset3
233480	7	421747	7	NULL	NULL	0	NULL	 10 & lt 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An arbitrary classification scheme was proposed based on the magnitude of deviation ( d ) as : additive ( & lt ; or = 10 % , class-I ) and moderately ( 10 & lt ; d & lt ; or = 30 % , class-II ) , highly ( 30 & lt ; d & lt ; or = 50 % , class-III ) and very highly ( ) 50 % , class-IV ) antagonistic/synergistic .
	manualset3
233481	8	421747	7	NULL	NULL	0	NULL	d & lt 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An arbitrary classification scheme was proposed based on the magnitude of deviation ( d ) as : additive ( & lt ; or = 10 % , class-I ) and moderately ( 10 & lt ; d & lt ; or = 30 % , class-II ) , highly ( 30 & lt ; d & lt ; or = 50 % , class-III ) and very highly ( ) 50 % , class-IV ) antagonistic/synergistic .
	manualset3
233482	9	421747	7	NULL	NULL	0	NULL	30 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An arbitrary classification scheme was proposed based on the magnitude of deviation ( d ) as : additive ( & lt ; or = 10 % , class-I ) and moderately ( 10 & lt ; d & lt ; or = 30 % , class-II ) , highly ( 30 & lt ; d & lt ; or = 50 % , class-III ) and very highly ( ) 50 % , class-IV ) antagonistic/synergistic .
	manualset3
233483	10	421747	7	NULL	NULL	0	NULL	class-II 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	An arbitrary classification scheme was proposed based on the magnitude of deviation ( d ) as : additive ( & lt ; or = 10 % , class-I ) and moderately ( 10 & lt ; d & lt ; or = 30 % , class-II ) , highly ( 30 & lt ; d & lt ; or = 50 % , class-III ) and very highly ( ) 50 % , class-IV ) antagonistic/synergistic .
	manualset3
233484	11	421747	7	NULL	NULL	0	NULL	 30	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	An arbitrary classification scheme was proposed based on the magnitude of deviation ( d ) as : additive ( & lt ; or = 10 % , class-I ) and moderately ( 10 & lt ; d & lt ; or = 30 % , class-II ) , highly ( 30 & lt ; d & lt ; or = 50 % , class-III ) and very highly ( ) 50 % , class-IV ) antagonistic/synergistic .
	manualset3
233485	12	421747	7	NULL	NULL	0	NULL	& lt	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An arbitrary classification scheme was proposed based on the magnitude of deviation ( d ) as : additive ( & lt ; or = 10 % , class-I ) and moderately ( 10 & lt ; d & lt ; or = 30 % , class-II ) , highly ( 30 & lt ; d & lt ; or = 50 % , class-III ) and very highly ( ) 50 % , class-IV ) antagonistic/synergistic .
	manualset3
233486	13	421747	7	NULL	NULL	0	NULL	d & lt 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An arbitrary classification scheme was proposed based on the magnitude of deviation ( d ) as : additive ( & lt ; or = 10 % , class-I ) and moderately ( 10 & lt ; d & lt ; or = 30 % , class-II ) , highly ( 30 & lt ; d & lt ; or = 50 % , class-III ) and very highly ( ) 50 % , class-IV ) antagonistic/synergistic .
	manualset3
233487	14	421747	7	NULL	NULL	0	NULL	50 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An arbitrary classification scheme was proposed based on the magnitude of deviation ( d ) as : additive ( & lt ; or = 10 % , class-I ) and moderately ( 10 & lt ; d & lt ; or = 30 % , class-II ) , highly ( 30 & lt ; d & lt ; or = 50 % , class-III ) and very highly ( ) 50 % , class-IV ) antagonistic/synergistic .
	manualset3
233488	15	421747	7	NULL	NULL	0	NULL	class-III	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	An arbitrary classification scheme was proposed based on the magnitude of deviation ( d ) as : additive ( & lt ; or = 10 % , class-I ) and moderately ( 10 & lt ; d & lt ; or = 30 % , class-II ) , highly ( 30 & lt ; d & lt ; or = 50 % , class-III ) and very highly ( ) 50 % , class-IV ) antagonistic/synergistic .
	manualset3
233489	16	421747	7	NULL	NULL	0	NULL	50 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An arbitrary classification scheme was proposed based on the magnitude of deviation ( d ) as : additive ( & lt ; or = 10 % , class-I ) and moderately ( 10 & lt ; d & lt ; or = 30 % , class-II ) , highly ( 30 & lt ; d & lt ; or = 50 % , class-III ) and very highly ( ) 50 % , class-IV ) antagonistic/synergistic .
	manualset3
233490	17	421747	7	NULL	NULL	0	NULL	class-IV	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	An arbitrary classification scheme was proposed based on the magnitude of deviation ( d ) as : additive ( & lt ; or = 10 % , class-I ) and moderately ( 10 & lt ; d & lt ; or = 30 % , class-II ) , highly ( 30 & lt ; d & lt ; or = 50 % , class-III ) and very highly ( ) 50 % , class-IV ) antagonistic/synergistic .
	manualset3
233491	1	421748	7	NULL	NULL	NULL	NULL	Axial slices	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Axial slices were obtained at the proximal quarter , the middle and the distal quarter of the forearm .
	manualset3
233492	2	421748	7	NULL	NULL	NULL	NULL	proximal quarter	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Axial slices were obtained at the proximal quarter , the middle and the distal quarter of the forearm .
	manualset3
233493	3	421748	7	NULL	NULL	0	NULL	 middle quarter 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Axial slices were obtained at the proximal quarter , the middle and the distal quarter of the forearm .
	manualset3
233494	4	421748	7	NULL	NULL	0	NULL	distal quarter	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Axial slices were obtained at the proximal quarter , the middle and the distal quarter of the forearm .
	manualset3
233495	5	421748	7	NULL	NULL	0	NULL	forearm	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Axial slices were obtained at the proximal quarter , the middle and the distal quarter of the forearm .
	manualset3
233496	1	421749	7	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support a substantive role for BK potentiation during ACE inhibitor-induced renal vasodilation in dogs maintained on a low-sodium diet , with a relatively greater effect on MBF compared to CBF .
	manualset3
233497	2	421749	7	NULL	NULL	0	NULL	substantive role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support a substantive role for BK potentiation during ACE inhibitor-induced renal vasodilation in dogs maintained on a low-sodium diet , with a relatively greater effect on MBF compared to CBF .
	manualset3
233498	3	421749	7	NULL	NULL	0	NULL	BK potentiation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support a substantive role for BK potentiation during ACE inhibitor-induced renal vasodilation in dogs maintained on a low-sodium diet , with a relatively greater effect on MBF compared to CBF .
	manualset3
233499	4	421749	7	NULL	NULL	0	NULL	ACE inhibitor-induced renal vasodilation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support a substantive role for BK potentiation during ACE inhibitor-induced renal vasodilation in dogs maintained on a low-sodium diet , with a relatively greater effect on MBF compared to CBF .
	manualset3
233500	5	421749	7	NULL	NULL	0	NULL	dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support a substantive role for BK potentiation during ACE inhibitor-induced renal vasodilation in dogs maintained on a low-sodium diet , with a relatively greater effect on MBF compared to CBF .
	manualset3
233501	6	421749	7	NULL	NULL	0	NULL	 low-sodium diet 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support a substantive role for BK potentiation during ACE inhibitor-induced renal vasodilation in dogs maintained on a low-sodium diet , with a relatively greater effect on MBF compared to CBF .
	manualset3
233502	7	421749	7	NULL	NULL	0	NULL	greater effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support a substantive role for BK potentiation during ACE inhibitor-induced renal vasodilation in dogs maintained on a low-sodium diet , with a relatively greater effect on MBF compared to CBF .
	manualset3
233503	8	421749	7	NULL	NULL	0	NULL	MBF 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support a substantive role for BK potentiation during ACE inhibitor-induced renal vasodilation in dogs maintained on a low-sodium diet , with a relatively greater effect on MBF compared to CBF .
	manualset3
233504	9	421749	7	NULL	NULL	0	NULL	CBF	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These data support a substantive role for BK potentiation during ACE inhibitor-induced renal vasodilation in dogs maintained on a low-sodium diet , with a relatively greater effect on MBF compared to CBF .
	manualset3
233505	1	421750	7	NULL	NULL	0	NULL	strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Some of the strains were resistant to high levels of gentamicin or streptomycin ( or both ) , and two produced beta-lactamase ( Bla + ) .
	manualset3
233506	2	421750	7	NULL	NULL	0	NULL	high levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some of the strains were resistant to high levels of gentamicin or streptomycin ( or both ) , and two produced beta-lactamase ( Bla + ) .
	manualset3
233507	3	421750	7	NULL	NULL	0	NULL	 gentamicin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Some of the strains were resistant to high levels of gentamicin or streptomycin ( or both ) , and two produced beta-lactamase ( Bla + ) .
	manualset3
233508	4	421750	7	NULL	NULL	0	NULL	streptomycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Some of the strains were resistant to high levels of gentamicin or streptomycin ( or both ) , and two produced beta-lactamase ( Bla + ) .
	manualset3
233509	5	421750	7	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Some of the strains were resistant to high levels of gentamicin or streptomycin ( or both ) , and two produced beta-lactamase ( Bla + ) .
	manualset3
233510	6	421750	7	NULL	NULL	0	NULL	beta-lactamase ( Bla + )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Some of the strains were resistant to high levels of gentamicin or streptomycin ( or both ) , and two produced beta-lactamase ( Bla + ) .
	manualset3
233511	1	421751	7	NULL	NULL	0	NULL	Expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of the truncated cadherin-11 in MDA-MB-435S human mammary carcinoma cells reduced their motility and promoted calcium-dependent cell aggregation , frequent cell contacts , and functional gap-junctions .
	manualset3
233512	2	421751	7	NULL	NULL	0	NULL	truncated cadherin-11	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of the truncated cadherin-11 in MDA-MB-435S human mammary carcinoma cells reduced their motility and promoted calcium-dependent cell aggregation , frequent cell contacts , and functional gap-junctions .
	manualset3
233513	3	421751	7	NULL	NULL	0	NULL	MDA-MB-435S human mammary carcinoma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of the truncated cadherin-11 in MDA-MB-435S human mammary carcinoma cells reduced their motility and promoted calcium-dependent cell aggregation , frequent cell contacts , and functional gap-junctions .
	manualset3
233514	4	421751	7	NULL	NULL	0	NULL	motility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of the truncated cadherin-11 in MDA-MB-435S human mammary carcinoma cells reduced their motility and promoted calcium-dependent cell aggregation , frequent cell contacts , and functional gap-junctions .
	manualset3
233515	5	421751	7	NULL	NULL	0	NULL	calcium-dependent cell aggregation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of the truncated cadherin-11 in MDA-MB-435S human mammary carcinoma cells reduced their motility and promoted calcium-dependent cell aggregation , frequent cell contacts , and functional gap-junctions .
	manualset3
233516	6	421751	7	NULL	NULL	0	NULL	cell contacts	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of the truncated cadherin-11 in MDA-MB-435S human mammary carcinoma cells reduced their motility and promoted calcium-dependent cell aggregation , frequent cell contacts , and functional gap-junctions .
	manualset3
233517	7	421751	7	NULL	NULL	0	NULL	functional gap-junctions 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression of the truncated cadherin-11 in MDA-MB-435S human mammary carcinoma cells reduced their motility and promoted calcium-dependent cell aggregation , frequent cell contacts , and functional gap-junctions .
	manualset3
233518	1	421752	7	NULL	NULL	0	NULL	Traction device	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Traction device to improve CT imaging of lower cervical spine .
	manualset3
233519	2	421752	7	NULL	NULL	0	NULL	 CT imaging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Traction device to improve CT imaging of lower cervical spine .
	manualset3
233520	3	421752	7	NULL	NULL	0	NULL	lower cervical spine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Traction device to improve CT imaging of lower cervical spine .
	manualset3
233521	1	421753	7	NULL	NULL	0	NULL	Learning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Learning from accident and error : avoiding the hazards of workload , stress , and routine interruptions in the emergency department .
	manualset3
233522	2	421753	7	NULL	NULL	0	NULL	accident	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Learning from accident and error : avoiding the hazards of workload , stress , and routine interruptions in the emergency department .
	manualset3
233523	3	421753	7	NULL	NULL	0	NULL	error	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Learning from accident and error : avoiding the hazards of workload , stress , and routine interruptions in the emergency department .
	manualset3
233524	4	421753	7	NULL	NULL	0	NULL	hazards	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Learning from accident and error : avoiding the hazards of workload , stress , and routine interruptions in the emergency department .
	manualset3
233525	5	421753	7	NULL	NULL	0	NULL	 workload	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Learning from accident and error : avoiding the hazards of workload , stress , and routine interruptions in the emergency department .
	manualset3
233526	6	421753	7	NULL	NULL	0	NULL	stress	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Learning from accident and error : avoiding the hazards of workload , stress , and routine interruptions in the emergency department .
	manualset3
233527	7	421753	7	NULL	NULL	0	NULL	routine interruptions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Learning from accident and error : avoiding the hazards of workload , stress , and routine interruptions in the emergency department .
	manualset3
233528	8	421753	7	NULL	NULL	0	NULL	emergency department	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Learning from accident and error : avoiding the hazards of workload , stress , and routine interruptions in the emergency department .
	manualset3
233798	1	421754	7	NULL	NULL	0	NULL	Communication	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Communication and behavior change for cancer control .
	manualset3
233799	2	421754	7	NULL	NULL	0	NULL	behavior change	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Communication and behavior change for cancer control .
	manualset3
233800	3	421754	7	NULL	NULL	0	NULL	cancer control	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Communication and behavior change for cancer control .
	manualset3
233801	1	421755	7	NULL	NULL	0	NULL	Vascular mediators	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Vascular mediators and factors other than classic T-cell-mediated rejection may play a role in this process , and aggressive multimodality therapy may improve survival .
	manualset3
233802	2	421755	7	NULL	NULL	0	NULL	 factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Vascular mediators and factors other than classic T-cell-mediated rejection may play a role in this process , and aggressive multimodality therapy may improve survival .
	manualset3
233803	3	421755	7	NULL	NULL	0	NULL	classic T-cell-mediated rejection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Vascular mediators and factors other than classic T-cell-mediated rejection may play a role in this process , and aggressive multimodality therapy may improve survival .
	manualset3
233804	4	421755	7	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Vascular mediators and factors other than classic T-cell-mediated rejection may play a role in this process , and aggressive multimodality therapy may improve survival .
	manualset3
233805	5	421755	7	NULL	NULL	0	NULL	process	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Vascular mediators and factors other than classic T-cell-mediated rejection may play a role in this process , and aggressive multimodality therapy may improve survival .
	manualset3
233806	6	421755	7	NULL	NULL	0	NULL	aggressive multimodality therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Vascular mediators and factors other than classic T-cell-mediated rejection may play a role in this process , and aggressive multimodality therapy may improve survival .
	manualset3
233807	7	421755	7	NULL	NULL	0	NULL	survival 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Vascular mediators and factors other than classic T-cell-mediated rejection may play a role in this process , and aggressive multimodality therapy may improve survival .
	manualset3
233808	1	421756	7	NULL	NULL	0	NULL	preparation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The preparation of the complex was tested and analyzed with regard to cellular damage by visible light activation .
	manualset3
233809	2	421756	7	NULL	NULL	0	NULL	complex 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The preparation of the complex was tested and analyzed with regard to cellular damage by visible light activation .
	manualset3
233810	3	421756	7	NULL	NULL	0	NULL	cellular damage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The preparation of the complex was tested and analyzed with regard to cellular damage by visible light activation .
	manualset3
233811	4	421756	7	NULL	NULL	0	NULL	visible light activation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The preparation of the complex was tested and analyzed with regard to cellular damage by visible light activation .
	manualset3
233812	1	421757	7	NULL	NULL	0	NULL	majority	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of prevention efforts offer services to individual parents , families , or children with the goal of altering those behaviors and attitudes that contribute to risk .
	manualset3
233813	2	421757	7	NULL	NULL	0	NULL	prevention efforts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of prevention efforts offer services to individual parents , families , or children with the goal of altering those behaviors and attitudes that contribute to risk .
	manualset3
233814	3	421757	7	NULL	NULL	0	NULL	individual parents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of prevention efforts offer services to individual parents , families , or children with the goal of altering those behaviors and attitudes that contribute to risk .
	manualset3
233815	4	421757	7	NULL	NULL	0	NULL	families	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of prevention efforts offer services to individual parents , families , or children with the goal of altering those behaviors and attitudes that contribute to risk .
	manualset3
233816	5	421757	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of prevention efforts offer services to individual parents , families , or children with the goal of altering those behaviors and attitudes that contribute to risk .
	manualset3
233817	6	421757	7	NULL	NULL	0	NULL	goal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of prevention efforts offer services to individual parents , families , or children with the goal of altering those behaviors and attitudes that contribute to risk .
	manualset3
233818	7	421757	7	NULL	NULL	0	NULL	behaviors	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of prevention efforts offer services to individual parents , families , or children with the goal of altering those behaviors and attitudes that contribute to risk .
	manualset3
233819	8	421757	7	NULL	NULL	0	NULL	attitudes	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of prevention efforts offer services to individual parents , families , or children with the goal of altering those behaviors and attitudes that contribute to risk .
	manualset3
233820	9	421757	7	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of prevention efforts offer services to individual parents , families , or children with the goal of altering those behaviors and attitudes that contribute to risk .
	manualset3
233821	10	421757	7	NULL	NULL	0	NULL	services	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The majority of prevention efforts offer services to individual parents , families , or children with the goal of altering those behaviors and attitudes that contribute to risk .
	manualset3
233822	1	421758	7	NULL	NULL	0	NULL	 authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors describe a patient with von Willebrand 's disease in whom pregnancy itself improved factor VIII activity , enabling performance of an epidural block for labor and delivery .
	manualset3
233823	2	421758	7	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors describe a patient with von Willebrand 's disease in whom pregnancy itself improved factor VIII activity , enabling performance of an epidural block for labor and delivery .
	manualset3
233824	3	421758	7	NULL	NULL	0	NULL	von Willebrand 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors describe a patient with von Willebrand 's disease in whom pregnancy itself improved factor VIII activity , enabling performance of an epidural block for labor and delivery .
	manualset3
233825	4	421758	7	NULL	NULL	0	NULL	pregnancy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors describe a patient with von Willebrand 's disease in whom pregnancy itself improved factor VIII activity , enabling performance of an epidural block for labor and delivery .
	manualset3
233826	5	421758	7	NULL	NULL	0	NULL	 factor VIII activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors describe a patient with von Willebrand 's disease in whom pregnancy itself improved factor VIII activity , enabling performance of an epidural block for labor and delivery .
	manualset3
233827	6	421758	7	NULL	NULL	0	NULL	performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors describe a patient with von Willebrand 's disease in whom pregnancy itself improved factor VIII activity , enabling performance of an epidural block for labor and delivery .
	manualset3
233828	7	421758	7	NULL	NULL	0	NULL	epidural block	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors describe a patient with von Willebrand 's disease in whom pregnancy itself improved factor VIII activity , enabling performance of an epidural block for labor and delivery .
	manualset3
233829	8	421758	7	NULL	NULL	0	NULL	 labor 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors describe a patient with von Willebrand 's disease in whom pregnancy itself improved factor VIII activity , enabling performance of an epidural block for labor and delivery .
	manualset3
233830	9	421758	7	NULL	NULL	0	NULL	delivery	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors describe a patient with von Willebrand 's disease in whom pregnancy itself improved factor VIII activity , enabling performance of an epidural block for labor and delivery .
	manualset3
233831	1	421759	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Some patients noted reduction of tonus and spasticity ; but others had no benefit , nor was the course of the disease altered by long-term administration of baclofen .
	manualset3
233832	2	421759	7	NULL	NULL	0	NULL	reduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Some patients noted reduction of tonus and spasticity ; but others had no benefit , nor was the course of the disease altered by long-term administration of baclofen .
	manualset3
233833	3	421759	7	NULL	NULL	0	NULL	tonus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Some patients noted reduction of tonus and spasticity ; but others had no benefit , nor was the course of the disease altered by long-term administration of baclofen .
	manualset3
233834	4	421759	7	NULL	NULL	0	NULL	 spasticity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Some patients noted reduction of tonus and spasticity ; but others had no benefit , nor was the course of the disease altered by long-term administration of baclofen .
	manualset3
233835	5	421759	7	NULL	NULL	0	NULL	course	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Some patients noted reduction of tonus and spasticity ; but others had no benefit , nor was the course of the disease altered by long-term administration of baclofen .
	manualset3
233836	6	421759	7	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Some patients noted reduction of tonus and spasticity ; but others had no benefit , nor was the course of the disease altered by long-term administration of baclofen .
	manualset3
233837	7	421759	7	NULL	NULL	0	NULL	 long-term administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Some patients noted reduction of tonus and spasticity ; but others had no benefit , nor was the course of the disease altered by long-term administration of baclofen .
	manualset3
233838	8	421759	7	NULL	NULL	0	NULL	baclofen	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Some patients noted reduction of tonus and spasticity ; but others had no benefit , nor was the course of the disease altered by long-term administration of baclofen .
	manualset3
233839	1	421760	7	NULL	NULL	0	NULL	 role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	To elucidate the role of CBP in the adult brain , we generated conditional knock-out ( cKO ) mice in which CBP is completely inactivated in excitatory neurons of the postnatal forebrain .
	manualset3
233840	2	421760	7	NULL	NULL	0	NULL	CBP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To elucidate the role of CBP in the adult brain , we generated conditional knock-out ( cKO ) mice in which CBP is completely inactivated in excitatory neurons of the postnatal forebrain .
	manualset3
233841	3	421760	7	NULL	NULL	0	NULL	adult brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To elucidate the role of CBP in the adult brain , we generated conditional knock-out ( cKO ) mice in which CBP is completely inactivated in excitatory neurons of the postnatal forebrain .
	manualset3
233842	4	421760	7	NULL	NULL	0	NULL	conditional knock-out ( cKO ) mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	To elucidate the role of CBP in the adult brain , we generated conditional knock-out ( cKO ) mice in which CBP is completely inactivated in excitatory neurons of the postnatal forebrain .
	manualset3
233843	5	421760	7	NULL	NULL	0	NULL	CBP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	To elucidate the role of CBP in the adult brain , we generated conditional knock-out ( cKO ) mice in which CBP is completely inactivated in excitatory neurons of the postnatal forebrain .
	manualset3
233844	6	421760	7	NULL	NULL	0	NULL	excitatory neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	To elucidate the role of CBP in the adult brain , we generated conditional knock-out ( cKO ) mice in which CBP is completely inactivated in excitatory neurons of the postnatal forebrain .
	manualset3
233845	7	421760	7	NULL	NULL	0	NULL	postnatal forebrain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	To elucidate the role of CBP in the adult brain , we generated conditional knock-out ( cKO ) mice in which CBP is completely inactivated in excitatory neurons of the postnatal forebrain .
	manualset3
233846	1	421761	7	NULL	NULL	0	NULL	Anti-TGF-beta treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-TGF-beta treatment of allogeneic transplant recipients with GVHD significantly decreased the histological evidence of pneumonitis at day 4 after HSV-1 infection .
	manualset3
233847	2	421761	7	NULL	NULL	0	NULL	allogeneic transplant recipients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-TGF-beta treatment of allogeneic transplant recipients with GVHD significantly decreased the histological evidence of pneumonitis at day 4 after HSV-1 infection .
	manualset3
233848	3	421761	7	NULL	NULL	0	NULL	GVHD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-TGF-beta treatment of allogeneic transplant recipients with GVHD significantly decreased the histological evidence of pneumonitis at day 4 after HSV-1 infection .
	manualset3
233849	4	421761	7	NULL	NULL	0	NULL	histological evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-TGF-beta treatment of allogeneic transplant recipients with GVHD significantly decreased the histological evidence of pneumonitis at day 4 after HSV-1 infection .
	manualset3
233850	5	421761	7	NULL	NULL	0	NULL	 pneumonitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-TGF-beta treatment of allogeneic transplant recipients with GVHD significantly decreased the histological evidence of pneumonitis at day 4 after HSV-1 infection .
	manualset3
233851	6	421761	7	NULL	NULL	0	NULL	day 4	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-TGF-beta treatment of allogeneic transplant recipients with GVHD significantly decreased the histological evidence of pneumonitis at day 4 after HSV-1 infection .
	manualset3
233852	7	421761	7	NULL	NULL	0	NULL	HSV-1 infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-TGF-beta treatment of allogeneic transplant recipients with GVHD significantly decreased the histological evidence of pneumonitis at day 4 after HSV-1 infection .
	manualset3
234885	1	421762	7	NULL	NULL	0	NULL	HBV-DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	HBV-DNA was detected in 9/78 ( 11.54 % ) of the anti-HBc-positive units , and thus , occult HBV infection was detected in 9/712 ( 1.26 % ) of the accepted blood donations .
	manualset3
234886	2	421762	7	NULL	NULL	0	NULL	 9/78	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	HBV-DNA was detected in 9/78 ( 11.54 % ) of the anti-HBc-positive units , and thus , occult HBV infection was detected in 9/712 ( 1.26 % ) of the accepted blood donations .
	manualset3
234887	3	421762	7	NULL	NULL	0	NULL	11.54 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	HBV-DNA was detected in 9/78 ( 11.54 % ) of the anti-HBc-positive units , and thus , occult HBV infection was detected in 9/712 ( 1.26 % ) of the accepted blood donations .
	manualset3
234888	4	421762	7	NULL	NULL	0	NULL	anti-HBc-positive units	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	HBV-DNA was detected in 9/78 ( 11.54 % ) of the anti-HBc-positive units , and thus , occult HBV infection was detected in 9/712 ( 1.26 % ) of the accepted blood donations .
	manualset3
234889	5	421762	7	NULL	NULL	0	NULL	occult HBV infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	HBV-DNA was detected in 9/78 ( 11.54 % ) of the anti-HBc-positive units , and thus , occult HBV infection was detected in 9/712 ( 1.26 % ) of the accepted blood donations .
	manualset3
234890	6	421762	7	NULL	NULL	NULL	NULL	9/712	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	HBV-DNA was detected in 9/78 ( 11.54 % ) of the anti-HBc-positive units , and thus , occult HBV infection was detected in 9/712 ( 1.26 % ) of the accepted blood donations .
	manualset3
234891	7	421762	7	NULL	NULL	0	NULL	1.26 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	HBV-DNA was detected in 9/78 ( 11.54 % ) of the anti-HBc-positive units , and thus , occult HBV infection was detected in 9/712 ( 1.26 % ) of the accepted blood donations .
	manualset3
234892	8	421762	7	NULL	NULL	0	NULL	accepted blood donations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	HBV-DNA was detected in 9/78 ( 11.54 % ) of the anti-HBc-positive units , and thus , occult HBV infection was detected in 9/712 ( 1.26 % ) of the accepted blood donations .
	manualset3
234893	1	421763	7	NULL	NULL	0	NULL	antibiotics 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Various antibiotics and bacterial pathogens are used as models to demonstrate the utility of PK/PD parameters in predicting the in vivo efficacy of antimicrobial therapy .
	manualset3
234894	2	421763	7	NULL	NULL	0	NULL	bacterial pathogens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Various antibiotics and bacterial pathogens are used as models to demonstrate the utility of PK/PD parameters in predicting the in vivo efficacy of antimicrobial therapy .
	manualset3
234895	3	421763	7	NULL	NULL	0	NULL	models 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Various antibiotics and bacterial pathogens are used as models to demonstrate the utility of PK/PD parameters in predicting the in vivo efficacy of antimicrobial therapy .
	manualset3
234896	4	421763	7	NULL	NULL	0	NULL	 utility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Various antibiotics and bacterial pathogens are used as models to demonstrate the utility of PK/PD parameters in predicting the in vivo efficacy of antimicrobial therapy .
	manualset3
234897	5	421763	7	NULL	NULL	0	NULL	PK/PD parameters	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Various antibiotics and bacterial pathogens are used as models to demonstrate the utility of PK/PD parameters in predicting the in vivo efficacy of antimicrobial therapy .
	manualset3
234898	6	421763	7	NULL	NULL	0	NULL	in vivo efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Various antibiotics and bacterial pathogens are used as models to demonstrate the utility of PK/PD parameters in predicting the in vivo efficacy of antimicrobial therapy .
	manualset3
234899	7	421763	7	NULL	NULL	0	NULL	antimicrobial therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Various antibiotics and bacterial pathogens are used as models to demonstrate the utility of PK/PD parameters in predicting the in vivo efficacy of antimicrobial therapy .
	manualset3
234900	1	421764	7	NULL	NULL	0	NULL	case 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( A case of Sertoli cell tumor of the testis with prostatic cancer ) .
	manualset3
234901	2	421764	7	NULL	NULL	0	NULL	Sertoli cell tumor	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( A case of Sertoli cell tumor of the testis with prostatic cancer ) .
	manualset3
234902	3	421764	7	NULL	NULL	0	NULL	testis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( A case of Sertoli cell tumor of the testis with prostatic cancer ) .
	manualset3
234903	4	421764	7	NULL	NULL	0	NULL	prostatic cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( A case of Sertoli cell tumor of the testis with prostatic cancer ) .
	manualset3
234904	1	421765	7	NULL	NULL	0	NULL	assessment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An assessment of dynamic autoregulation from spontaneous fluctuations of cerebral blood flow velocity : a comparison of two models , index of autoregulation and mean flow index .
	manualset3
234905	2	421765	7	NULL	NULL	0	NULL	dynamic autoregulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An assessment of dynamic autoregulation from spontaneous fluctuations of cerebral blood flow velocity : a comparison of two models , index of autoregulation and mean flow index .
	manualset3
234906	3	421765	7	NULL	NULL	0	NULL	 spontaneous fluctuations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An assessment of dynamic autoregulation from spontaneous fluctuations of cerebral blood flow velocity : a comparison of two models , index of autoregulation and mean flow index .
	manualset3
234907	4	421765	7	NULL	NULL	0	NULL	cerebral blood flow velocity 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An assessment of dynamic autoregulation from spontaneous fluctuations of cerebral blood flow velocity : a comparison of two models , index of autoregulation and mean flow index .
	manualset3
234908	5	421765	7	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	An assessment of dynamic autoregulation from spontaneous fluctuations of cerebral blood flow velocity : a comparison of two models , index of autoregulation and mean flow index .
	manualset3
234909	6	421765	7	NULL	NULL	0	NULL	two models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	An assessment of dynamic autoregulation from spontaneous fluctuations of cerebral blood flow velocity : a comparison of two models , index of autoregulation and mean flow index .
	manualset3
234910	7	421765	7	NULL	NULL	0	NULL	index	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An assessment of dynamic autoregulation from spontaneous fluctuations of cerebral blood flow velocity : a comparison of two models , index of autoregulation and mean flow index .
	manualset3
234911	8	421765	7	NULL	NULL	0	NULL	autoregulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An assessment of dynamic autoregulation from spontaneous fluctuations of cerebral blood flow velocity : a comparison of two models , index of autoregulation and mean flow index .
	manualset3
234912	9	421765	7	NULL	NULL	0	NULL	mean flow index	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An assessment of dynamic autoregulation from spontaneous fluctuations of cerebral blood flow velocity : a comparison of two models , index of autoregulation and mean flow index .
	manualset3
234913	1	421766	7	NULL	NULL	0	NULL	Consumers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Consumers and payers demand quality care at a significantly reduced price .
	manualset3
234914	2	421766	7	NULL	NULL	NULL	NULL	payers 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Consumers and payers demand quality care at a significantly reduced price .
	manualset3
234915	3	421766	7	NULL	NULL	0	NULL	reduced price	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Consumers and payers demand quality care at a significantly reduced price .
	manualset3
234916	1	421767	7	NULL	NULL	0	NULL	crystal 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal , mol-ecules are linked by N-HO hydrogen bonds involving the N-H and C = O groups of the amide function , leading to a chain along ( -101 ) .
	manualset3
234917	2	421767	7	NULL	NULL	0	NULL	mol-ecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal , mol-ecules are linked by N-HO hydrogen bonds involving the N-H and C = O groups of the amide function , leading to a chain along ( -101 ) .
	manualset3
234918	3	421767	7	NULL	NULL	0	NULL	N-HO hydrogen bonds	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal , mol-ecules are linked by N-HO hydrogen bonds involving the N-H and C = O groups of the amide function , leading to a chain along ( -101 ) .
	manualset3
234919	4	421767	7	NULL	NULL	0	NULL	N-H groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal , mol-ecules are linked by N-HO hydrogen bonds involving the N-H and C = O groups of the amide function , leading to a chain along ( -101 ) .
	manualset3
234920	5	421767	7	NULL	NULL	0	NULL	C = O groups 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal , mol-ecules are linked by N-HO hydrogen bonds involving the N-H and C = O groups of the amide function , leading to a chain along ( -101 ) .
	manualset3
234921	6	421767	7	NULL	NULL	0	NULL	amide function 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal , mol-ecules are linked by N-HO hydrogen bonds involving the N-H and C = O groups of the amide function , leading to a chain along ( -101 ) .
	manualset3
234922	7	421767	7	NULL	NULL	0	NULL	chain	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal , mol-ecules are linked by N-HO hydrogen bonds involving the N-H and C = O groups of the amide function , leading to a chain along ( -101 ) .
	manualset3
234923	8	421767	7	NULL	NULL	0	NULL	 -101	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In the crystal , mol-ecules are linked by N-HO hydrogen bonds involving the N-H and C = O groups of the amide function , leading to a chain along ( -101 ) .
	manualset3
234924	1	421768	7	NULL	NULL	0	NULL	inability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The inability of the respiratory burst to result in the binding of phenacetin to nucleic acid suggests that arylamides are not normally activated or metabolized by activated granulocytes .
	manualset3
234925	2	421768	7	NULL	NULL	0	NULL	 respiratory burst	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The inability of the respiratory burst to result in the binding of phenacetin to nucleic acid suggests that arylamides are not normally activated or metabolized by activated granulocytes .
	manualset3
234926	3	421768	7	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The inability of the respiratory burst to result in the binding of phenacetin to nucleic acid suggests that arylamides are not normally activated or metabolized by activated granulocytes .
	manualset3
234927	4	421768	7	NULL	NULL	0	NULL	phenacetin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The inability of the respiratory burst to result in the binding of phenacetin to nucleic acid suggests that arylamides are not normally activated or metabolized by activated granulocytes .
	manualset3
234928	5	421768	7	NULL	NULL	0	NULL	nucleic acid	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The inability of the respiratory burst to result in the binding of phenacetin to nucleic acid suggests that arylamides are not normally activated or metabolized by activated granulocytes .
	manualset3
234929	6	421768	7	NULL	NULL	0	NULL	arylamides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The inability of the respiratory burst to result in the binding of phenacetin to nucleic acid suggests that arylamides are not normally activated or metabolized by activated granulocytes .
	manualset3
234930	7	421768	7	NULL	NULL	0	NULL	activated granulocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The inability of the respiratory burst to result in the binding of phenacetin to nucleic acid suggests that arylamides are not normally activated or metabolized by activated granulocytes .
	manualset3
234931	1	421769	7	NULL	NULL	0	NULL	Studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of specific properties of tumor cell membranes using stereoscan microscopy .
	manualset3
234932	2	421769	7	NULL	NULL	NULL	NULL	specific properties	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Studies of specific properties of tumor cell membranes using stereoscan microscopy .
	manualset3
234933	3	421769	7	NULL	NULL	0	NULL	tumor cell membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies of specific properties of tumor cell membranes using stereoscan microscopy .
	manualset3
234934	4	421769	7	NULL	NULL	NULL	NULL	stereoscan microscopy	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Studies of specific properties of tumor cell membranes using stereoscan microscopy .
	manualset3
234935	1	421770	7	NULL	NULL	0	NULL	PRA values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Their PRA values declined after DTT treatment on average from 96.2 % to 45 % and from 95 % to 52.5 % , respectively .
	manualset3
234936	2	421770	7	NULL	NULL	0	NULL	DTT treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Their PRA values declined after DTT treatment on average from 96.2 % to 45 % and from 95 % to 52.5 % , respectively .
	manualset3
234937	3	421770	7	NULL	NULL	0	NULL	96.2 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Their PRA values declined after DTT treatment on average from 96.2 % to 45 % and from 95 % to 52.5 % , respectively .
	manualset3
234938	4	421770	7	NULL	NULL	0	NULL	45 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Their PRA values declined after DTT treatment on average from 96.2 % to 45 % and from 95 % to 52.5 % , respectively .
	manualset3
234939	5	421770	7	NULL	NULL	0	NULL	 95 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Their PRA values declined after DTT treatment on average from 96.2 % to 45 % and from 95 % to 52.5 % , respectively .
	manualset3
234940	6	421770	7	NULL	NULL	0	NULL	52.5 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Their PRA values declined after DTT treatment on average from 96.2 % to 45 % and from 95 % to 52.5 % , respectively .
	manualset3
239463	7	421770	7	NULL	NULL	0	NULL	average	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Their PRA values declined after DTT treatment on average from 96.2 % to 45 % and from 95 % to 52.5 % , respectively .
	manualset3
234941	1	421771	7	NULL	NULL	0	NULL	astounding number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An astounding number of biologic agents are currently in development for the treatment of IBD and other immune-mediated conditions .
	manualset3
234942	2	421771	7	NULL	NULL	0	NULL	biologic agents 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An astounding number of biologic agents are currently in development for the treatment of IBD and other immune-mediated conditions .
	manualset3
234943	3	421771	7	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An astounding number of biologic agents are currently in development for the treatment of IBD and other immune-mediated conditions .
	manualset3
234944	4	421771	7	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An astounding number of biologic agents are currently in development for the treatment of IBD and other immune-mediated conditions .
	manualset3
234945	5	421771	7	NULL	NULL	0	NULL	IBD 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	An astounding number of biologic agents are currently in development for the treatment of IBD and other immune-mediated conditions .
	manualset3
234946	6	421771	7	NULL	NULL	0	NULL	immune-mediated conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An astounding number of biologic agents are currently in development for the treatment of IBD and other immune-mediated conditions .
	manualset3
234947	1	421772	7	NULL	NULL	0	NULL	diabetic women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among diabetic women , the significantly higher prevalence of deficiency was observed only in the young age group ( p less than 0.005 ) , whereas the difference among the older age group was not significant ( p greater than 0.1 ) .
	manualset3
234948	2	421772	7	NULL	NULL	0	NULL	deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among diabetic women , the significantly higher prevalence of deficiency was observed only in the young age group ( p less than 0.005 ) , whereas the difference among the older age group was not significant ( p greater than 0.1 ) .
	manualset3
234949	3	421772	7	NULL	NULL	0	NULL	young age group 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among diabetic women , the significantly higher prevalence of deficiency was observed only in the young age group ( p less than 0.005 ) , whereas the difference among the older age group was not significant ( p greater than 0.1 ) .
	manualset3
234950	4	421772	7	NULL	NULL	0	NULL	p less than 0.005	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among diabetic women , the significantly higher prevalence of deficiency was observed only in the young age group ( p less than 0.005 ) , whereas the difference among the older age group was not significant ( p greater than 0.1 ) .
	manualset3
234951	5	421772	7	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Among diabetic women , the significantly higher prevalence of deficiency was observed only in the young age group ( p less than 0.005 ) , whereas the difference among the older age group was not significant ( p greater than 0.1 ) .
	manualset3
234952	6	421772	7	NULL	NULL	0	NULL	older age group 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among diabetic women , the significantly higher prevalence of deficiency was observed only in the young age group ( p less than 0.005 ) , whereas the difference among the older age group was not significant ( p greater than 0.1 ) .
	manualset3
234953	7	421772	7	NULL	NULL	0	NULL	p greater than 0.1	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Among diabetic women , the significantly higher prevalence of deficiency was observed only in the young age group ( p less than 0.005 ) , whereas the difference among the older age group was not significant ( p greater than 0.1 ) .
	manualset3
239464	8	421772	7	NULL	NULL	0	NULL	higher prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among diabetic women , the significantly higher prevalence of deficiency was observed only in the young age group ( p less than 0.005 ) , whereas the difference among the older age group was not significant ( p greater than 0.1 ) .
	manualset3
234954	1	421773	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients were examined pre - and postoperatively by roentgenography , endoscopy , gastric acid analysis , and serum gastrin evaluation .
	manualset3
234955	2	421773	7	NULL	NULL	NULL	NULL	roentgenography	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	All patients were examined pre - and postoperatively by roentgenography , endoscopy , gastric acid analysis , and serum gastrin evaluation .
	manualset3
234956	3	421773	7	NULL	NULL	0	NULL	endoscopy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients were examined pre - and postoperatively by roentgenography , endoscopy , gastric acid analysis , and serum gastrin evaluation .
	manualset3
234957	4	421773	7	NULL	NULL	0	NULL	gastric acid analysis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients were examined pre - and postoperatively by roentgenography , endoscopy , gastric acid analysis , and serum gastrin evaluation .
	manualset3
234958	5	421773	7	NULL	NULL	0	NULL	serum gastrin evaluation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients were examined pre - and postoperatively by roentgenography , endoscopy , gastric acid analysis , and serum gastrin evaluation .
	manualset3
234959	1	421774	7	NULL	NULL	0	NULL	DA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , DA markedly decreased all components of the synaptic responses evoked by electrical stimulation of layer I or VI , and in particular the monosynaptic excitatory postsynaptic potential ( EPSP ) which arises from activation of glutamatergic receptors .
	manualset3
234960	2	421774	7	NULL	NULL	0	NULL	components	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , DA markedly decreased all components of the synaptic responses evoked by electrical stimulation of layer I or VI , and in particular the monosynaptic excitatory postsynaptic potential ( EPSP ) which arises from activation of glutamatergic receptors .
	manualset3
234961	3	421774	7	NULL	NULL	0	NULL	 synaptic responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , DA markedly decreased all components of the synaptic responses evoked by electrical stimulation of layer I or VI , and in particular the monosynaptic excitatory postsynaptic potential ( EPSP ) which arises from activation of glutamatergic receptors .
	manualset3
234962	4	421774	7	NULL	NULL	0	NULL	electrical stimulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , DA markedly decreased all components of the synaptic responses evoked by electrical stimulation of layer I or VI , and in particular the monosynaptic excitatory postsynaptic potential ( EPSP ) which arises from activation of glutamatergic receptors .
	manualset3
234963	5	421774	7	NULL	NULL	0	NULL	layer I	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , DA markedly decreased all components of the synaptic responses evoked by electrical stimulation of layer I or VI , and in particular the monosynaptic excitatory postsynaptic potential ( EPSP ) which arises from activation of glutamatergic receptors .
	manualset3
234964	6	421774	7	NULL	NULL	0	NULL	layer VI 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , DA markedly decreased all components of the synaptic responses evoked by electrical stimulation of layer I or VI , and in particular the monosynaptic excitatory postsynaptic potential ( EPSP ) which arises from activation of glutamatergic receptors .
	manualset3
234965	7	421774	7	NULL	NULL	0	NULL	monosynaptic excitatory postsynaptic potential ( EPSP )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , DA markedly decreased all components of the synaptic responses evoked by electrical stimulation of layer I or VI , and in particular the monosynaptic excitatory postsynaptic potential ( EPSP ) which arises from activation of glutamatergic receptors .
	manualset3
234966	8	421774	7	NULL	NULL	NULL	NULL	activation 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In contrast , DA markedly decreased all components of the synaptic responses evoked by electrical stimulation of layer I or VI , and in particular the monosynaptic excitatory postsynaptic potential ( EPSP ) which arises from activation of glutamatergic receptors .
	manualset3
234967	9	421774	7	NULL	NULL	0	NULL	glutamatergic receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , DA markedly decreased all components of the synaptic responses evoked by electrical stimulation of layer I or VI , and in particular the monosynaptic excitatory postsynaptic potential ( EPSP ) which arises from activation of glutamatergic receptors .
	manualset3
234968	1	421775	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This study of three samples of california adults aged sixty and over confirms the relevance of an equity frame-of-reference in accounting for the satisfaction of older people with specific conditions of their lives and with their overall life satisfaction or sense of well-being
	manualset3
234969	2	421775	7	NULL	NULL	0	NULL	 three samples 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This study of three samples of california adults aged sixty and over confirms the relevance of an equity frame-of-reference in accounting for the satisfaction of older people with specific conditions of their lives and with their overall life satisfaction or sense of well-being
	manualset3
234970	3	421775	7	NULL	NULL	0	NULL	california adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This study of three samples of california adults aged sixty and over confirms the relevance of an equity frame-of-reference in accounting for the satisfaction of older people with specific conditions of their lives and with their overall life satisfaction or sense of well-being
	manualset3
234971	4	421775	7	NULL	NULL	0	NULL	sixty	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	This study of three samples of california adults aged sixty and over confirms the relevance of an equity frame-of-reference in accounting for the satisfaction of older people with specific conditions of their lives and with their overall life satisfaction or sense of well-being
	manualset3
234972	5	421775	7	NULL	NULL	0	NULL	equity frame-of-reference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This study of three samples of california adults aged sixty and over confirms the relevance of an equity frame-of-reference in accounting for the satisfaction of older people with specific conditions of their lives and with their overall life satisfaction or sense of well-being
	manualset3
234973	6	421775	7	NULL	NULL	0	NULL	satisfaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This study of three samples of california adults aged sixty and over confirms the relevance of an equity frame-of-reference in accounting for the satisfaction of older people with specific conditions of their lives and with their overall life satisfaction or sense of well-being
	manualset3
234974	7	421775	7	NULL	NULL	0	NULL	older people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This study of three samples of california adults aged sixty and over confirms the relevance of an equity frame-of-reference in accounting for the satisfaction of older people with specific conditions of their lives and with their overall life satisfaction or sense of well-being
	manualset3
234975	8	421775	7	NULL	NULL	0	NULL	specific conditions 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	This study of three samples of california adults aged sixty and over confirms the relevance of an equity frame-of-reference in accounting for the satisfaction of older people with specific conditions of their lives and with their overall life satisfaction or sense of well-being
	manualset3
234976	9	421775	7	NULL	NULL	0	NULL	lives 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This study of three samples of california adults aged sixty and over confirms the relevance of an equity frame-of-reference in accounting for the satisfaction of older people with specific conditions of their lives and with their overall life satisfaction or sense of well-being
	manualset3
234977	10	421775	7	NULL	NULL	0	NULL	overall life satisfaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This study of three samples of california adults aged sixty and over confirms the relevance of an equity frame-of-reference in accounting for the satisfaction of older people with specific conditions of their lives and with their overall life satisfaction or sense of well-being
	manualset3
234978	11	421775	7	NULL	NULL	0	NULL	sense of well-being	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This study of three samples of california adults aged sixty and over confirms the relevance of an equity frame-of-reference in accounting for the satisfaction of older people with specific conditions of their lives and with their overall life satisfaction or sense of well-being
	manualset3
234979	1	421776	7	NULL	NULL	NULL	NULL	Separation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Separation and biological properties of Phaseolus vulgaris isolectins .
	manualset3
234980	2	421776	7	NULL	NULL	0	NULL	 biological properties	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Separation and biological properties of Phaseolus vulgaris isolectins .
	manualset3
234981	3	421776	7	NULL	NULL	0	NULL	Phaseolus vulgaris isolectins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Separation and biological properties of Phaseolus vulgaris isolectins .
	manualset3
234982	1	421777	7	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	By comparison with a vascular reference , labeled red cells , a set of interstitial materials are found to enter the Disse space in a delayed-wave , flow-limited fashion , larger materials being excluded from a proportion of the space , and labeled water is found to undergo flow-limited distribution into the liver cells .
	manualset3
234983	2	421777	7	NULL	NULL	0	NULL	vascular reference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	By comparison with a vascular reference , labeled red cells , a set of interstitial materials are found to enter the Disse space in a delayed-wave , flow-limited fashion , larger materials being excluded from a proportion of the space , and labeled water is found to undergo flow-limited distribution into the liver cells .
	manualset3
234984	3	421777	7	NULL	NULL	0	NULL	labeled red cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	By comparison with a vascular reference , labeled red cells , a set of interstitial materials are found to enter the Disse space in a delayed-wave , flow-limited fashion , larger materials being excluded from a proportion of the space , and labeled water is found to undergo flow-limited distribution into the liver cells .
	manualset3
234985	4	421777	7	NULL	NULL	0	NULL	set	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	By comparison with a vascular reference , labeled red cells , a set of interstitial materials are found to enter the Disse space in a delayed-wave , flow-limited fashion , larger materials being excluded from a proportion of the space , and labeled water is found to undergo flow-limited distribution into the liver cells .
	manualset3
234986	5	421777	7	NULL	NULL	0	NULL	interstitial materials	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	By comparison with a vascular reference , labeled red cells , a set of interstitial materials are found to enter the Disse space in a delayed-wave , flow-limited fashion , larger materials being excluded from a proportion of the space , and labeled water is found to undergo flow-limited distribution into the liver cells .
	manualset3
234987	6	421777	7	NULL	NULL	0	NULL	Disse space	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	By comparison with a vascular reference , labeled red cells , a set of interstitial materials are found to enter the Disse space in a delayed-wave , flow-limited fashion , larger materials being excluded from a proportion of the space , and labeled water is found to undergo flow-limited distribution into the liver cells .
	manualset3
234988	7	421777	7	NULL	NULL	0	NULL	delayed-wave 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	By comparison with a vascular reference , labeled red cells , a set of interstitial materials are found to enter the Disse space in a delayed-wave , flow-limited fashion , larger materials being excluded from a proportion of the space , and labeled water is found to undergo flow-limited distribution into the liver cells .
	manualset3
234989	8	421777	7	NULL	NULL	0	NULL	flow-limited fashion	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	By comparison with a vascular reference , labeled red cells , a set of interstitial materials are found to enter the Disse space in a delayed-wave , flow-limited fashion , larger materials being excluded from a proportion of the space , and labeled water is found to undergo flow-limited distribution into the liver cells .
	manualset3
234990	9	421777	7	NULL	NULL	0	NULL	larger materials	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	By comparison with a vascular reference , labeled red cells , a set of interstitial materials are found to enter the Disse space in a delayed-wave , flow-limited fashion , larger materials being excluded from a proportion of the space , and labeled water is found to undergo flow-limited distribution into the liver cells .
	manualset3
234991	10	421777	7	NULL	NULL	0	NULL	proportion	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	By comparison with a vascular reference , labeled red cells , a set of interstitial materials are found to enter the Disse space in a delayed-wave , flow-limited fashion , larger materials being excluded from a proportion of the space , and labeled water is found to undergo flow-limited distribution into the liver cells .
	manualset3
234992	11	421777	7	NULL	NULL	0	NULL	space	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	By comparison with a vascular reference , labeled red cells , a set of interstitial materials are found to enter the Disse space in a delayed-wave , flow-limited fashion , larger materials being excluded from a proportion of the space , and labeled water is found to undergo flow-limited distribution into the liver cells .
	manualset3
234993	12	421777	7	NULL	NULL	0	NULL	labeled water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	By comparison with a vascular reference , labeled red cells , a set of interstitial materials are found to enter the Disse space in a delayed-wave , flow-limited fashion , larger materials being excluded from a proportion of the space , and labeled water is found to undergo flow-limited distribution into the liver cells .
	manualset3
234994	13	421777	7	NULL	NULL	0	NULL	flow-limited distribution 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	By comparison with a vascular reference , labeled red cells , a set of interstitial materials are found to enter the Disse space in a delayed-wave , flow-limited fashion , larger materials being excluded from a proportion of the space , and labeled water is found to undergo flow-limited distribution into the liver cells .
	manualset3
234995	14	421777	7	NULL	NULL	0	NULL	liver cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	By comparison with a vascular reference , labeled red cells , a set of interstitial materials are found to enter the Disse space in a delayed-wave , flow-limited fashion , larger materials being excluded from a proportion of the space , and labeled water is found to undergo flow-limited distribution into the liver cells .
	manualset3
234996	1	421778	7	NULL	NULL	0	NULL	 mutagenesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	By applying mutagenesis and intergeneric protoplast fusion , we have obtained a recombinant strain ( Tahrir-25 ) that overproduced cellulases ( exo -- 1 , 4-glucanase , endo -- 1 , 4-glucanase and -1 , 4 - glucosidase ) that facilitated complete cellulolysis of agricultural residues .
	manualset3
234997	2	421778	7	NULL	NULL	0	NULL	 intergeneric protoplast fusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	By applying mutagenesis and intergeneric protoplast fusion , we have obtained a recombinant strain ( Tahrir-25 ) that overproduced cellulases ( exo -- 1 , 4-glucanase , endo -- 1 , 4-glucanase and -1 , 4 - glucosidase ) that facilitated complete cellulolysis of agricultural residues .
	manualset3
234998	3	421778	7	NULL	NULL	0	NULL	recombinant strain ( Tahrir-25 )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	By applying mutagenesis and intergeneric protoplast fusion , we have obtained a recombinant strain ( Tahrir-25 ) that overproduced cellulases ( exo -- 1 , 4-glucanase , endo -- 1 , 4-glucanase and -1 , 4 - glucosidase ) that facilitated complete cellulolysis of agricultural residues .
	manualset3
234999	4	421778	7	NULL	NULL	0	NULL	cellulases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	By applying mutagenesis and intergeneric protoplast fusion , we have obtained a recombinant strain ( Tahrir-25 ) that overproduced cellulases ( exo -- 1 , 4-glucanase , endo -- 1 , 4-glucanase and -1 , 4 - glucosidase ) that facilitated complete cellulolysis of agricultural residues .
	manualset3
235000	5	421778	7	NULL	NULL	0	NULL	 exo -- 1 , 4-glucanase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	By applying mutagenesis and intergeneric protoplast fusion , we have obtained a recombinant strain ( Tahrir-25 ) that overproduced cellulases ( exo -- 1 , 4-glucanase , endo -- 1 , 4-glucanase and -1 , 4 - glucosidase ) that facilitated complete cellulolysis of agricultural residues .
	manualset3
235001	6	421778	7	NULL	NULL	0	NULL	endo -- 1 , 4-glucanase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	By applying mutagenesis and intergeneric protoplast fusion , we have obtained a recombinant strain ( Tahrir-25 ) that overproduced cellulases ( exo -- 1 , 4-glucanase , endo -- 1 , 4-glucanase and -1 , 4 - glucosidase ) that facilitated complete cellulolysis of agricultural residues .
	manualset3
235002	7	421778	7	NULL	NULL	0	NULL	-1 , 4 - glucosidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	By applying mutagenesis and intergeneric protoplast fusion , we have obtained a recombinant strain ( Tahrir-25 ) that overproduced cellulases ( exo -- 1 , 4-glucanase , endo -- 1 , 4-glucanase and -1 , 4 - glucosidase ) that facilitated complete cellulolysis of agricultural residues .
	manualset3
235003	8	421778	7	NULL	NULL	0	NULL	complete cellulolysis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	By applying mutagenesis and intergeneric protoplast fusion , we have obtained a recombinant strain ( Tahrir-25 ) that overproduced cellulases ( exo -- 1 , 4-glucanase , endo -- 1 , 4-glucanase and -1 , 4 - glucosidase ) that facilitated complete cellulolysis of agricultural residues .
	manualset3
235004	9	421778	7	NULL	NULL	0	NULL	agricultural residues	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	By applying mutagenesis and intergeneric protoplast fusion , we have obtained a recombinant strain ( Tahrir-25 ) that overproduced cellulases ( exo -- 1 , 4-glucanase , endo -- 1 , 4-glucanase and -1 , 4 - glucosidase ) that facilitated complete cellulolysis of agricultural residues .
	manualset3
235005	1	421779	7	NULL	NULL	0	NULL	knock-out mutants	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	We now show that knock-out mutants of either nrdD or nrdG can not grow during strict anaerobiosis , achieved by inclusion of sodium sulfide in the medium .
	manualset3
235006	2	421779	7	NULL	NULL	0	NULL	nrdD	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	We now show that knock-out mutants of either nrdD or nrdG can not grow during strict anaerobiosis , achieved by inclusion of sodium sulfide in the medium .
	manualset3
235007	3	421779	7	NULL	NULL	0	NULL	 nrdG	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	We now show that knock-out mutants of either nrdD or nrdG can not grow during strict anaerobiosis , achieved by inclusion of sodium sulfide in the medium .
	manualset3
235008	4	421779	7	NULL	NULL	0	NULL	anaerobiosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We now show that knock-out mutants of either nrdD or nrdG can not grow during strict anaerobiosis , achieved by inclusion of sodium sulfide in the medium .
	manualset3
235009	5	421779	7	NULL	NULL	0	NULL	 inclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We now show that knock-out mutants of either nrdD or nrdG can not grow during strict anaerobiosis , achieved by inclusion of sodium sulfide in the medium .
	manualset3
235010	6	421779	7	NULL	NULL	0	NULL	sodium sulfide 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We now show that knock-out mutants of either nrdD or nrdG can not grow during strict anaerobiosis , achieved by inclusion of sodium sulfide in the medium .
	manualset3
235011	7	421779	7	NULL	NULL	0	NULL	medium	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We now show that knock-out mutants of either nrdD or nrdG can not grow during strict anaerobiosis , achieved by inclusion of sodium sulfide in the medium .
	manualset3
235012	1	421780	7	NULL	NULL	0	NULL	One week	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	One week later , startle was measured in response to 30 air-puff stimuli for each rat .
	manualset3
235013	2	421780	7	NULL	NULL	0	NULL	30 air-puff stimuli	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	One week later , startle was measured in response to 30 air-puff stimuli for each rat .
	manualset3
235014	3	421780	7	NULL	NULL	0	NULL	 rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	One week later , startle was measured in response to 30 air-puff stimuli for each rat .
	manualset3
235218	4	421780	7	NULL	NULL	0	NULL	startle	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	One week later , startle was measured in response to 30 air-puff stimuli for each rat .
	manualset3
235219	1	421781	7	NULL	NULL	0	NULL	fitness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We measured the fitness of offspring in a common garden at the warm-edge species range limit .
	manualset3
235220	2	421781	7	NULL	NULL	NULL	NULL	offspring	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We measured the fitness of offspring in a common garden at the warm-edge species range limit .
	manualset3
235221	3	421781	7	NULL	NULL	0	NULL	garden	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	We measured the fitness of offspring in a common garden at the warm-edge species range limit .
	manualset3
235222	4	421781	7	NULL	NULL	0	NULL	warm-edge species range limit	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We measured the fitness of offspring in a common garden at the warm-edge species range limit .
	manualset3
235223	1	421782	7	NULL	NULL	0	NULL	drug treatments 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Current drug treatments for ASDs and the related disorders -- fragile X syndrome ( FXS ) and Rett syndrome -- target specific symptoms but do not address the basic underlying etiologies .
	manualset3
235224	2	421782	7	NULL	NULL	0	NULL	ASDs	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Current drug treatments for ASDs and the related disorders -- fragile X syndrome ( FXS ) and Rett syndrome -- target specific symptoms but do not address the basic underlying etiologies .
	manualset3
235225	3	421782	7	NULL	NULL	0	NULL	disorders 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Current drug treatments for ASDs and the related disorders -- fragile X syndrome ( FXS ) and Rett syndrome -- target specific symptoms but do not address the basic underlying etiologies .
	manualset3
235226	4	421782	7	NULL	NULL	0	NULL	fragile X syndrome ( FXS ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Current drug treatments for ASDs and the related disorders -- fragile X syndrome ( FXS ) and Rett syndrome -- target specific symptoms but do not address the basic underlying etiologies .
	manualset3
235227	5	421782	7	NULL	NULL	0	NULL	Rett syndrome 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Current drug treatments for ASDs and the related disorders -- fragile X syndrome ( FXS ) and Rett syndrome -- target specific symptoms but do not address the basic underlying etiologies .
	manualset3
235228	6	421782	7	NULL	NULL	0	NULL	target specific symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Current drug treatments for ASDs and the related disorders -- fragile X syndrome ( FXS ) and Rett syndrome -- target specific symptoms but do not address the basic underlying etiologies .
	manualset3
235229	7	421782	7	NULL	NULL	0	NULL	etiologies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Current drug treatments for ASDs and the related disorders -- fragile X syndrome ( FXS ) and Rett syndrome -- target specific symptoms but do not address the basic underlying etiologies .
	manualset3
235230	1	421783	7	NULL	NULL	0	NULL	levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It increased further the levels of PGE2 , nitrite and tumor necrosis factor in the culture supernatant of the macrophages induced by the supernatant from concanavalin A-stimulated spleen cell cultures .
	manualset3
235231	2	421783	7	NULL	NULL	0	NULL	PGE2	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It increased further the levels of PGE2 , nitrite and tumor necrosis factor in the culture supernatant of the macrophages induced by the supernatant from concanavalin A-stimulated spleen cell cultures .
	manualset3
235232	3	421783	7	NULL	NULL	0	NULL	 nitrite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It increased further the levels of PGE2 , nitrite and tumor necrosis factor in the culture supernatant of the macrophages induced by the supernatant from concanavalin A-stimulated spleen cell cultures .
	manualset3
235233	4	421783	7	NULL	NULL	0	NULL	tumor necrosis factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	It increased further the levels of PGE2 , nitrite and tumor necrosis factor in the culture supernatant of the macrophages induced by the supernatant from concanavalin A-stimulated spleen cell cultures .
	manualset3
235234	5	421783	7	NULL	NULL	NULL	NULL	culture supernatant 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It increased further the levels of PGE2 , nitrite and tumor necrosis factor in the culture supernatant of the macrophages induced by the supernatant from concanavalin A-stimulated spleen cell cultures .
	manualset3
235235	6	421783	7	NULL	NULL	0	NULL	macrophages 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It increased further the levels of PGE2 , nitrite and tumor necrosis factor in the culture supernatant of the macrophages induced by the supernatant from concanavalin A-stimulated spleen cell cultures .
	manualset3
235236	8	421783	7	NULL	NULL	NULL	NULL	concanavalin A-stimulated spleen cell cultures	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It increased further the levels of PGE2 , nitrite and tumor necrosis factor in the culture supernatant of the macrophages induced by the supernatant from concanavalin A-stimulated spleen cell cultures .
	manualset3
235237	7	421783	7	NULL	NULL	0	NULL	supernatant	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It increased further the levels of PGE2 , nitrite and tumor necrosis factor in the culture supernatant of the macrophages induced by the supernatant from concanavalin A-stimulated spleen cell cultures .
	manualset3
235238	1	421784	7	NULL	NULL	0	NULL	purpose 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the present study was to directly test the influence of eicosapentaenoic acid ( 20 : 5 n-3 ) and docosahexaenoic acid ( 22 : 6 n-3 ) in the sn-2 position of phosphatidylcholine ( PC ) on the activity of LCAT .
	manualset3
235239	2	421784	7	NULL	NULL	0	NULL	present study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the present study was to directly test the influence of eicosapentaenoic acid ( 20 : 5 n-3 ) and docosahexaenoic acid ( 22 : 6 n-3 ) in the sn-2 position of phosphatidylcholine ( PC ) on the activity of LCAT .
	manualset3
235240	3	421784	7	NULL	NULL	0	NULL	influence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the present study was to directly test the influence of eicosapentaenoic acid ( 20 : 5 n-3 ) and docosahexaenoic acid ( 22 : 6 n-3 ) in the sn-2 position of phosphatidylcholine ( PC ) on the activity of LCAT .
	manualset3
235241	4	421784	7	NULL	NULL	0	NULL	eicosapentaenoic acid ( 20 : 5 n-3 )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the present study was to directly test the influence of eicosapentaenoic acid ( 20 : 5 n-3 ) and docosahexaenoic acid ( 22 : 6 n-3 ) in the sn-2 position of phosphatidylcholine ( PC ) on the activity of LCAT .
	manualset3
235242	5	421784	7	NULL	NULL	0	NULL	docosahexaenoic acid ( 22 : 6 n-3 )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the present study was to directly test the influence of eicosapentaenoic acid ( 20 : 5 n-3 ) and docosahexaenoic acid ( 22 : 6 n-3 ) in the sn-2 position of phosphatidylcholine ( PC ) on the activity of LCAT .
	manualset3
235243	6	421784	7	NULL	NULL	0	NULL	sn-2 position	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the present study was to directly test the influence of eicosapentaenoic acid ( 20 : 5 n-3 ) and docosahexaenoic acid ( 22 : 6 n-3 ) in the sn-2 position of phosphatidylcholine ( PC ) on the activity of LCAT .
	manualset3
235244	7	421784	7	NULL	NULL	0	NULL	phosphatidylcholine ( PC ) 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the present study was to directly test the influence of eicosapentaenoic acid ( 20 : 5 n-3 ) and docosahexaenoic acid ( 22 : 6 n-3 ) in the sn-2 position of phosphatidylcholine ( PC ) on the activity of LCAT .
	manualset3
235245	8	421784	7	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the present study was to directly test the influence of eicosapentaenoic acid ( 20 : 5 n-3 ) and docosahexaenoic acid ( 22 : 6 n-3 ) in the sn-2 position of phosphatidylcholine ( PC ) on the activity of LCAT .
	manualset3
235246	9	421784	7	NULL	NULL	0	NULL	LCAT	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The purpose of the present study was to directly test the influence of eicosapentaenoic acid ( 20 : 5 n-3 ) and docosahexaenoic acid ( 22 : 6 n-3 ) in the sn-2 position of phosphatidylcholine ( PC ) on the activity of LCAT .
	manualset3
235247	1	421785	7	NULL	NULL	0	NULL	association 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The association of lactational changes in the breasts with primary lymphoma of the brain has not been reported .
	manualset3
235248	2	421785	7	NULL	NULL	0	NULL	lactational changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The association of lactational changes in the breasts with primary lymphoma of the brain has not been reported .
	manualset3
235249	3	421785	7	NULL	NULL	0	NULL	breasts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The association of lactational changes in the breasts with primary lymphoma of the brain has not been reported .
	manualset3
235250	4	421785	7	NULL	NULL	0	NULL	primary lymphoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The association of lactational changes in the breasts with primary lymphoma of the brain has not been reported .
	manualset3
235251	5	421785	7	NULL	NULL	0	NULL	brain 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The association of lactational changes in the breasts with primary lymphoma of the brain has not been reported .
	manualset3
235252	1	421786	7	NULL	NULL	0	NULL	Case histories	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Case histories of maritime basins in the Mediterranean , Caribbean , and Pacific show that the demographic structure of small islands has been particularly sensitive to changing economic opportunities , the vagaries of market forces , and cataclysmic natural events .
	manualset3
235253	2	421786	7	NULL	NULL	NULL	NULL	maritime basins	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Case histories of maritime basins in the Mediterranean , Caribbean , and Pacific show that the demographic structure of small islands has been particularly sensitive to changing economic opportunities , the vagaries of market forces , and cataclysmic natural events .
	manualset3
235254	3	421786	7	NULL	NULL	NULL	NULL	Mediterranean 	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Case histories of maritime basins in the Mediterranean , Caribbean , and Pacific show that the demographic structure of small islands has been particularly sensitive to changing economic opportunities , the vagaries of market forces , and cataclysmic natural events .
	manualset3
235255	4	421786	7	NULL	NULL	NULL	NULL	Caribbean	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Case histories of maritime basins in the Mediterranean , Caribbean , and Pacific show that the demographic structure of small islands has been particularly sensitive to changing economic opportunities , the vagaries of market forces , and cataclysmic natural events .
	manualset3
235256	5	421786	7	NULL	NULL	NULL	NULL	Pacific	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Case histories of maritime basins in the Mediterranean , Caribbean , and Pacific show that the demographic structure of small islands has been particularly sensitive to changing economic opportunities , the vagaries of market forces , and cataclysmic natural events .
	manualset3
235257	6	421786	7	NULL	NULL	0	NULL	demographic structure	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Case histories of maritime basins in the Mediterranean , Caribbean , and Pacific show that the demographic structure of small islands has been particularly sensitive to changing economic opportunities , the vagaries of market forces , and cataclysmic natural events .
	manualset3
235258	7	421786	7	NULL	NULL	0	NULL	small islands	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Case histories of maritime basins in the Mediterranean , Caribbean , and Pacific show that the demographic structure of small islands has been particularly sensitive to changing economic opportunities , the vagaries of market forces , and cataclysmic natural events .
	manualset3
235259	8	421786	7	NULL	NULL	0	NULL	economic opportunities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Case histories of maritime basins in the Mediterranean , Caribbean , and Pacific show that the demographic structure of small islands has been particularly sensitive to changing economic opportunities , the vagaries of market forces , and cataclysmic natural events .
	manualset3
235260	9	421786	7	NULL	NULL	0	NULL	 vagaries	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Case histories of maritime basins in the Mediterranean , Caribbean , and Pacific show that the demographic structure of small islands has been particularly sensitive to changing economic opportunities , the vagaries of market forces , and cataclysmic natural events .
	manualset3
235261	10	421786	7	NULL	NULL	0	NULL	market forces	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Case histories of maritime basins in the Mediterranean , Caribbean , and Pacific show that the demographic structure of small islands has been particularly sensitive to changing economic opportunities , the vagaries of market forces , and cataclysmic natural events .
	manualset3
235262	11	421786	7	NULL	NULL	NULL	NULL	cataclysmic natural events .	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Case histories of maritime basins in the Mediterranean , Caribbean , and Pacific show that the demographic structure of small islands has been particularly sensitive to changing economic opportunities , the vagaries of market forces , and cataclysmic natural events .
	manualset3
235263	1	421787	7	NULL	NULL	0	NULL	Effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of hypothalamic deafferentation and estrogen on the distribution and content of hypothalamic LHRH ( author 's transl ) ) .
	manualset3
235264	2	421787	7	NULL	NULL	0	NULL	hypothalamic deafferentation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of hypothalamic deafferentation and estrogen on the distribution and content of hypothalamic LHRH ( author 's transl ) ) .
	manualset3
235265	3	421787	7	NULL	NULL	0	NULL	estrogen 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of hypothalamic deafferentation and estrogen on the distribution and content of hypothalamic LHRH ( author 's transl ) ) .
	manualset3
235266	4	421787	7	NULL	NULL	0	NULL	distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of hypothalamic deafferentation and estrogen on the distribution and content of hypothalamic LHRH ( author 's transl ) ) .
	manualset3
235267	5	421787	7	NULL	NULL	0	NULL	content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of hypothalamic deafferentation and estrogen on the distribution and content of hypothalamic LHRH ( author 's transl ) ) .
	manualset3
235268	6	421787	7	NULL	NULL	0	NULL	hypothalamic LHRH 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of hypothalamic deafferentation and estrogen on the distribution and content of hypothalamic LHRH ( author 's transl ) ) .
	manualset3
235269	7	421787	7	NULL	NULL	0	NULL	 author 's transl	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of hypothalamic deafferentation and estrogen on the distribution and content of hypothalamic LHRH ( author 's transl ) ) .
	manualset3
235270	1	421788	7	NULL	NULL	0	NULL	HLA system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	HLA system and its association to chronic hepatitis and persistence of HBsAg in the organism .
	manualset3
235271	2	421788	7	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	HLA system and its association to chronic hepatitis and persistence of HBsAg in the organism .
	manualset3
235272	3	421788	7	NULL	NULL	0	NULL	chronic hepatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	HLA system and its association to chronic hepatitis and persistence of HBsAg in the organism .
	manualset3
235273	4	421788	7	NULL	NULL	0	NULL	HBsAg	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	HLA system and its association to chronic hepatitis and persistence of HBsAg in the organism .
	manualset3
235274	5	421788	7	NULL	NULL	0	NULL	organism	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	HLA system and its association to chronic hepatitis and persistence of HBsAg in the organism .
	manualset3
235275	1	421789	7	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to further explore this hypothesis we have studied insulin action , binding , and degradation in freshly isolated hepatocytes from rats rendered insulin resistant by the administration of dexamethasone , 1.0 mg/kg every other day , for 1 and 4 wk , and in dexamethasone-treated ( 0.1 muM for 24 h ) primary cultures of hepatocytes from normal rats .
	manualset3
235276	2	421789	7	NULL	NULL	0	NULL	insulin action	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to further explore this hypothesis we have studied insulin action , binding , and degradation in freshly isolated hepatocytes from rats rendered insulin resistant by the administration of dexamethasone , 1.0 mg/kg every other day , for 1 and 4 wk , and in dexamethasone-treated ( 0.1 muM for 24 h ) primary cultures of hepatocytes from normal rats .
	manualset3
235277	3	421789	7	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to further explore this hypothesis we have studied insulin action , binding , and degradation in freshly isolated hepatocytes from rats rendered insulin resistant by the administration of dexamethasone , 1.0 mg/kg every other day , for 1 and 4 wk , and in dexamethasone-treated ( 0.1 muM for 24 h ) primary cultures of hepatocytes from normal rats .
	manualset3
235278	4	421789	7	NULL	NULL	0	NULL	degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to further explore this hypothesis we have studied insulin action , binding , and degradation in freshly isolated hepatocytes from rats rendered insulin resistant by the administration of dexamethasone , 1.0 mg/kg every other day , for 1 and 4 wk , and in dexamethasone-treated ( 0.1 muM for 24 h ) primary cultures of hepatocytes from normal rats .
	manualset3
235279	5	421789	7	NULL	NULL	0	NULL	freshly isolated hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to further explore this hypothesis we have studied insulin action , binding , and degradation in freshly isolated hepatocytes from rats rendered insulin resistant by the administration of dexamethasone , 1.0 mg/kg every other day , for 1 and 4 wk , and in dexamethasone-treated ( 0.1 muM for 24 h ) primary cultures of hepatocytes from normal rats .
	manualset3
235280	6	421789	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to further explore this hypothesis we have studied insulin action , binding , and degradation in freshly isolated hepatocytes from rats rendered insulin resistant by the administration of dexamethasone , 1.0 mg/kg every other day , for 1 and 4 wk , and in dexamethasone-treated ( 0.1 muM for 24 h ) primary cultures of hepatocytes from normal rats .
	manualset3
235281	7	421789	7	NULL	NULL	0	NULL	administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to further explore this hypothesis we have studied insulin action , binding , and degradation in freshly isolated hepatocytes from rats rendered insulin resistant by the administration of dexamethasone , 1.0 mg/kg every other day , for 1 and 4 wk , and in dexamethasone-treated ( 0.1 muM for 24 h ) primary cultures of hepatocytes from normal rats .
	manualset3
235282	8	421789	7	NULL	NULL	0	NULL	dexamethasone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to further explore this hypothesis we have studied insulin action , binding , and degradation in freshly isolated hepatocytes from rats rendered insulin resistant by the administration of dexamethasone , 1.0 mg/kg every other day , for 1 and 4 wk , and in dexamethasone-treated ( 0.1 muM for 24 h ) primary cultures of hepatocytes from normal rats .
	manualset3
235283	9	421789	7	NULL	NULL	0	NULL	1.0 mg/kg	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to further explore this hypothesis we have studied insulin action , binding , and degradation in freshly isolated hepatocytes from rats rendered insulin resistant by the administration of dexamethasone , 1.0 mg/kg every other day , for 1 and 4 wk , and in dexamethasone-treated ( 0.1 muM for 24 h ) primary cultures of hepatocytes from normal rats .
	manualset3
235284	10	421789	7	NULL	NULL	0	NULL	day	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to further explore this hypothesis we have studied insulin action , binding , and degradation in freshly isolated hepatocytes from rats rendered insulin resistant by the administration of dexamethasone , 1.0 mg/kg every other day , for 1 and 4 wk , and in dexamethasone-treated ( 0.1 muM for 24 h ) primary cultures of hepatocytes from normal rats .
	manualset3
235285	11	421789	7	NULL	NULL	0	NULL	 1 wk	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to further explore this hypothesis we have studied insulin action , binding , and degradation in freshly isolated hepatocytes from rats rendered insulin resistant by the administration of dexamethasone , 1.0 mg/kg every other day , for 1 and 4 wk , and in dexamethasone-treated ( 0.1 muM for 24 h ) primary cultures of hepatocytes from normal rats .
	manualset3
235286	12	421789	7	NULL	NULL	0	NULL	4 wk	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to further explore this hypothesis we have studied insulin action , binding , and degradation in freshly isolated hepatocytes from rats rendered insulin resistant by the administration of dexamethasone , 1.0 mg/kg every other day , for 1 and 4 wk , and in dexamethasone-treated ( 0.1 muM for 24 h ) primary cultures of hepatocytes from normal rats .
	manualset3
235287	13	421789	7	NULL	NULL	0	NULL	dexamethasone-treated primary cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to further explore this hypothesis we have studied insulin action , binding , and degradation in freshly isolated hepatocytes from rats rendered insulin resistant by the administration of dexamethasone , 1.0 mg/kg every other day , for 1 and 4 wk , and in dexamethasone-treated ( 0.1 muM for 24 h ) primary cultures of hepatocytes from normal rats .
	manualset3
235288	14	421789	7	NULL	NULL	0	NULL	 0.1 muM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to further explore this hypothesis we have studied insulin action , binding , and degradation in freshly isolated hepatocytes from rats rendered insulin resistant by the administration of dexamethasone , 1.0 mg/kg every other day , for 1 and 4 wk , and in dexamethasone-treated ( 0.1 muM for 24 h ) primary cultures of hepatocytes from normal rats .
	manualset3
235289	15	421789	7	NULL	NULL	0	NULL	hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to further explore this hypothesis we have studied insulin action , binding , and degradation in freshly isolated hepatocytes from rats rendered insulin resistant by the administration of dexamethasone , 1.0 mg/kg every other day , for 1 and 4 wk , and in dexamethasone-treated ( 0.1 muM for 24 h ) primary cultures of hepatocytes from normal rats .
	manualset3
235290	16	421789	7	NULL	NULL	0	NULL	normal rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to further explore this hypothesis we have studied insulin action , binding , and degradation in freshly isolated hepatocytes from rats rendered insulin resistant by the administration of dexamethasone , 1.0 mg/kg every other day , for 1 and 4 wk , and in dexamethasone-treated ( 0.1 muM for 24 h ) primary cultures of hepatocytes from normal rats .
	manualset3
235291	17	421789	7	NULL	NULL	0	NULL	 24 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In an attempt to further explore this hypothesis we have studied insulin action , binding , and degradation in freshly isolated hepatocytes from rats rendered insulin resistant by the administration of dexamethasone , 1.0 mg/kg every other day , for 1 and 4 wk , and in dexamethasone-treated ( 0.1 muM for 24 h ) primary cultures of hepatocytes from normal rats .
	manualset3
235292	1	421790	7	NULL	NULL	0	NULL	formation rates	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation rates of the main metabolites of the VP enantiomers were estimated in an in vitro intestinal microsomal study .
	manualset3
235293	2	421790	7	NULL	NULL	0	NULL	main metabolites 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation rates of the main metabolites of the VP enantiomers were estimated in an in vitro intestinal microsomal study .
	manualset3
235294	3	421790	7	NULL	NULL	0	NULL	VP enantiomers	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation rates of the main metabolites of the VP enantiomers were estimated in an in vitro intestinal microsomal study .
	manualset3
235295	4	421790	7	NULL	NULL	0	NULL	 in vitro intestinal microsomal study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The formation rates of the main metabolites of the VP enantiomers were estimated in an in vitro intestinal microsomal study .
	manualset3
235296	1	421791	7	NULL	NULL	0	NULL	attractive option	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An attractive option for Wiskott-Aldrich syndrome is gene therapy , which leads to complete cure .
	manualset3
235297	2	421791	7	NULL	NULL	0	NULL	Wiskott-Aldrich syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	An attractive option for Wiskott-Aldrich syndrome is gene therapy , which leads to complete cure .
	manualset3
235298	3	421791	7	NULL	NULL	0	NULL	gene therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An attractive option for Wiskott-Aldrich syndrome is gene therapy , which leads to complete cure .
	manualset3
235299	4	421791	7	NULL	NULL	0	NULL	cure 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An attractive option for Wiskott-Aldrich syndrome is gene therapy , which leads to complete cure .
	manualset3
235300	1	421792	7	NULL	NULL	0	NULL	( HSSSO ( 3 ) ) ( - )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	From ( HSSSO ( 3 ) ) ( - ) the longer chain sulfane monosulfonate ions ( HS ( n ) SO ( 3 ) ) ( - ) are formed by a series of sulfur transfer reactions , and these ions eventually split off homocyclic sulfur molecules S ( n ) .
	manualset3
235301	2	421792	7	NULL	NULL	0	NULL	longer chain sulfane monosulfonate ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	From ( HSSSO ( 3 ) ) ( - ) the longer chain sulfane monosulfonate ions ( HS ( n ) SO ( 3 ) ) ( - ) are formed by a series of sulfur transfer reactions , and these ions eventually split off homocyclic sulfur molecules S ( n ) .
	manualset3
235302	3	421792	7	NULL	NULL	0	NULL	( HS ( n ) SO ( 3 ) ) ( - ) 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	From ( HSSSO ( 3 ) ) ( - ) the longer chain sulfane monosulfonate ions ( HS ( n ) SO ( 3 ) ) ( - ) are formed by a series of sulfur transfer reactions , and these ions eventually split off homocyclic sulfur molecules S ( n ) .
	manualset3
235303	4	421792	7	NULL	NULL	0	NULL	series 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	From ( HSSSO ( 3 ) ) ( - ) the longer chain sulfane monosulfonate ions ( HS ( n ) SO ( 3 ) ) ( - ) are formed by a series of sulfur transfer reactions , and these ions eventually split off homocyclic sulfur molecules S ( n ) .
	manualset3
235304	5	421792	7	NULL	NULL	0	NULL	sulfur transfer reactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	From ( HSSSO ( 3 ) ) ( - ) the longer chain sulfane monosulfonate ions ( HS ( n ) SO ( 3 ) ) ( - ) are formed by a series of sulfur transfer reactions , and these ions eventually split off homocyclic sulfur molecules S ( n ) .
	manualset3
235305	6	421792	7	NULL	NULL	0	NULL	 ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	From ( HSSSO ( 3 ) ) ( - ) the longer chain sulfane monosulfonate ions ( HS ( n ) SO ( 3 ) ) ( - ) are formed by a series of sulfur transfer reactions , and these ions eventually split off homocyclic sulfur molecules S ( n ) .
	manualset3
235306	7	421792	7	NULL	NULL	0	NULL	homocyclic sulfur molecules S ( n )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	From ( HSSSO ( 3 ) ) ( - ) the longer chain sulfane monosulfonate ions ( HS ( n ) SO ( 3 ) ) ( - ) are formed by a series of sulfur transfer reactions , and these ions eventually split off homocyclic sulfur molecules S ( n ) .
	manualset3
235307	1	421793	7	NULL	NULL	0	NULL	adducts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Besides the adducts fac - ( ReX ( CO ) ( 3 ) ( H ( 2 ) L ) ) , in which the rhenium is coordinated to three carbonyl groups , the X anion , and the N , S-bidentate thiosemicarbazone ligand , the following complexes were also isolated : fac - ( ReBr ( CO ) ( 3 ) ( Hpyz ( B ) ) ) , the tetrameric complexes fac - ( Re ( pyz ( A ) ) ( CO ) ( 3 ) ) ( 4 ) and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ) ( 4 ) , and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ( H ( 2 ) O ) ) ( where Hpyz ( A ) and Hpyz ( B ) are pyrazolones derived by cyclization of H ( 2 ) L ( A ) and H ( 2 ) L ( B ) , respectively ) .
	manualset3
235308	2	421793	7	NULL	NULL	0	NULL	fac - ( ReX ( CO ) ( 3 ) ( H ( 2 ) L ) )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Besides the adducts fac - ( ReX ( CO ) ( 3 ) ( H ( 2 ) L ) ) , in which the rhenium is coordinated to three carbonyl groups , the X anion , and the N , S-bidentate thiosemicarbazone ligand , the following complexes were also isolated : fac - ( ReBr ( CO ) ( 3 ) ( Hpyz ( B ) ) ) , the tetrameric complexes fac - ( Re ( pyz ( A ) ) ( CO ) ( 3 ) ) ( 4 ) and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ) ( 4 ) , and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ( H ( 2 ) O ) ) ( where Hpyz ( A ) and Hpyz ( B ) are pyrazolones derived by cyclization of H ( 2 ) L ( A ) and H ( 2 ) L ( B ) , respectively ) .
	manualset3
235309	3	421793	7	NULL	NULL	0	NULL	 rhenium 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Besides the adducts fac - ( ReX ( CO ) ( 3 ) ( H ( 2 ) L ) ) , in which the rhenium is coordinated to three carbonyl groups , the X anion , and the N , S-bidentate thiosemicarbazone ligand , the following complexes were also isolated : fac - ( ReBr ( CO ) ( 3 ) ( Hpyz ( B ) ) ) , the tetrameric complexes fac - ( Re ( pyz ( A ) ) ( CO ) ( 3 ) ) ( 4 ) and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ) ( 4 ) , and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ( H ( 2 ) O ) ) ( where Hpyz ( A ) and Hpyz ( B ) are pyrazolones derived by cyclization of H ( 2 ) L ( A ) and H ( 2 ) L ( B ) , respectively ) .
	manualset3
235310	4	421793	7	NULL	NULL	0	NULL	 three carbonyl groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Besides the adducts fac - ( ReX ( CO ) ( 3 ) ( H ( 2 ) L ) ) , in which the rhenium is coordinated to three carbonyl groups , the X anion , and the N , S-bidentate thiosemicarbazone ligand , the following complexes were also isolated : fac - ( ReBr ( CO ) ( 3 ) ( Hpyz ( B ) ) ) , the tetrameric complexes fac - ( Re ( pyz ( A ) ) ( CO ) ( 3 ) ) ( 4 ) and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ) ( 4 ) , and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ( H ( 2 ) O ) ) ( where Hpyz ( A ) and Hpyz ( B ) are pyrazolones derived by cyclization of H ( 2 ) L ( A ) and H ( 2 ) L ( B ) , respectively ) .
	manualset3
235311	5	421793	7	NULL	NULL	0	NULL	X anion	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Besides the adducts fac - ( ReX ( CO ) ( 3 ) ( H ( 2 ) L ) ) , in which the rhenium is coordinated to three carbonyl groups , the X anion , and the N , S-bidentate thiosemicarbazone ligand , the following complexes were also isolated : fac - ( ReBr ( CO ) ( 3 ) ( Hpyz ( B ) ) ) , the tetrameric complexes fac - ( Re ( pyz ( A ) ) ( CO ) ( 3 ) ) ( 4 ) and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ) ( 4 ) , and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ( H ( 2 ) O ) ) ( where Hpyz ( A ) and Hpyz ( B ) are pyrazolones derived by cyclization of H ( 2 ) L ( A ) and H ( 2 ) L ( B ) , respectively ) .
	manualset3
235312	6	421793	7	NULL	NULL	0	NULL	N , S-bidentate thiosemicarbazone ligand	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Besides the adducts fac - ( ReX ( CO ) ( 3 ) ( H ( 2 ) L ) ) , in which the rhenium is coordinated to three carbonyl groups , the X anion , and the N , S-bidentate thiosemicarbazone ligand , the following complexes were also isolated : fac - ( ReBr ( CO ) ( 3 ) ( Hpyz ( B ) ) ) , the tetrameric complexes fac - ( Re ( pyz ( A ) ) ( CO ) ( 3 ) ) ( 4 ) and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ) ( 4 ) , and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ( H ( 2 ) O ) ) ( where Hpyz ( A ) and Hpyz ( B ) are pyrazolones derived by cyclization of H ( 2 ) L ( A ) and H ( 2 ) L ( B ) , respectively ) .
	manualset3
235313	7	421793	7	NULL	NULL	0	NULL	complexes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Besides the adducts fac - ( ReX ( CO ) ( 3 ) ( H ( 2 ) L ) ) , in which the rhenium is coordinated to three carbonyl groups , the X anion , and the N , S-bidentate thiosemicarbazone ligand , the following complexes were also isolated : fac - ( ReBr ( CO ) ( 3 ) ( Hpyz ( B ) ) ) , the tetrameric complexes fac - ( Re ( pyz ( A ) ) ( CO ) ( 3 ) ) ( 4 ) and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ) ( 4 ) , and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ( H ( 2 ) O ) ) ( where Hpyz ( A ) and Hpyz ( B ) are pyrazolones derived by cyclization of H ( 2 ) L ( A ) and H ( 2 ) L ( B ) , respectively ) .
	manualset3
235314	8	421793	7	NULL	NULL	0	NULL	 fac - ( ReBr ( CO ) ( 3 ) ( Hpyz ( B ) ) )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Besides the adducts fac - ( ReX ( CO ) ( 3 ) ( H ( 2 ) L ) ) , in which the rhenium is coordinated to three carbonyl groups , the X anion , and the N , S-bidentate thiosemicarbazone ligand , the following complexes were also isolated : fac - ( ReBr ( CO ) ( 3 ) ( Hpyz ( B ) ) ) , the tetrameric complexes fac - ( Re ( pyz ( A ) ) ( CO ) ( 3 ) ) ( 4 ) and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ) ( 4 ) , and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ( H ( 2 ) O ) ) ( where Hpyz ( A ) and Hpyz ( B ) are pyrazolones derived by cyclization of H ( 2 ) L ( A ) and H ( 2 ) L ( B ) , respectively ) .
	manualset3
235315	9	421793	7	NULL	NULL	0	NULL	tetrameric complexes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Besides the adducts fac - ( ReX ( CO ) ( 3 ) ( H ( 2 ) L ) ) , in which the rhenium is coordinated to three carbonyl groups , the X anion , and the N , S-bidentate thiosemicarbazone ligand , the following complexes were also isolated : fac - ( ReBr ( CO ) ( 3 ) ( Hpyz ( B ) ) ) , the tetrameric complexes fac - ( Re ( pyz ( A ) ) ( CO ) ( 3 ) ) ( 4 ) and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ) ( 4 ) , and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ( H ( 2 ) O ) ) ( where Hpyz ( A ) and Hpyz ( B ) are pyrazolones derived by cyclization of H ( 2 ) L ( A ) and H ( 2 ) L ( B ) , respectively ) .
	manualset3
235316	10	421793	7	NULL	NULL	0	NULL	fac - ( Re ( pyz ( A ) ) ( CO ) ( 3 ) ) ( 4 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Besides the adducts fac - ( ReX ( CO ) ( 3 ) ( H ( 2 ) L ) ) , in which the rhenium is coordinated to three carbonyl groups , the X anion , and the N , S-bidentate thiosemicarbazone ligand , the following complexes were also isolated : fac - ( ReBr ( CO ) ( 3 ) ( Hpyz ( B ) ) ) , the tetrameric complexes fac - ( Re ( pyz ( A ) ) ( CO ) ( 3 ) ) ( 4 ) and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ) ( 4 ) , and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ( H ( 2 ) O ) ) ( where Hpyz ( A ) and Hpyz ( B ) are pyrazolones derived by cyclization of H ( 2 ) L ( A ) and H ( 2 ) L ( B ) , respectively ) .
	manualset3
235317	11	421793	7	NULL	NULL	0	NULL	 fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ) ( 4 ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Besides the adducts fac - ( ReX ( CO ) ( 3 ) ( H ( 2 ) L ) ) , in which the rhenium is coordinated to three carbonyl groups , the X anion , and the N , S-bidentate thiosemicarbazone ligand , the following complexes were also isolated : fac - ( ReBr ( CO ) ( 3 ) ( Hpyz ( B ) ) ) , the tetrameric complexes fac - ( Re ( pyz ( A ) ) ( CO ) ( 3 ) ) ( 4 ) and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ) ( 4 ) , and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ( H ( 2 ) O ) ) ( where Hpyz ( A ) and Hpyz ( B ) are pyrazolones derived by cyclization of H ( 2 ) L ( A ) and H ( 2 ) L ( B ) , respectively ) .
	manualset3
235318	12	421793	7	NULL	NULL	0	NULL	fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ( H ( 2 ) O ) ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Besides the adducts fac - ( ReX ( CO ) ( 3 ) ( H ( 2 ) L ) ) , in which the rhenium is coordinated to three carbonyl groups , the X anion , and the N , S-bidentate thiosemicarbazone ligand , the following complexes were also isolated : fac - ( ReBr ( CO ) ( 3 ) ( Hpyz ( B ) ) ) , the tetrameric complexes fac - ( Re ( pyz ( A ) ) ( CO ) ( 3 ) ) ( 4 ) and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ) ( 4 ) , and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ( H ( 2 ) O ) ) ( where Hpyz ( A ) and Hpyz ( B ) are pyrazolones derived by cyclization of H ( 2 ) L ( A ) and H ( 2 ) L ( B ) , respectively ) .
	manualset3
235319	13	421793	7	NULL	NULL	0	NULL	Hpyz ( A )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Besides the adducts fac - ( ReX ( CO ) ( 3 ) ( H ( 2 ) L ) ) , in which the rhenium is coordinated to three carbonyl groups , the X anion , and the N , S-bidentate thiosemicarbazone ligand , the following complexes were also isolated : fac - ( ReBr ( CO ) ( 3 ) ( Hpyz ( B ) ) ) , the tetrameric complexes fac - ( Re ( pyz ( A ) ) ( CO ) ( 3 ) ) ( 4 ) and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ) ( 4 ) , and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ( H ( 2 ) O ) ) ( where Hpyz ( A ) and Hpyz ( B ) are pyrazolones derived by cyclization of H ( 2 ) L ( A ) and H ( 2 ) L ( B ) , respectively ) .
	manualset3
235320	14	421793	7	NULL	NULL	0	NULL	Hpyz ( B )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Besides the adducts fac - ( ReX ( CO ) ( 3 ) ( H ( 2 ) L ) ) , in which the rhenium is coordinated to three carbonyl groups , the X anion , and the N , S-bidentate thiosemicarbazone ligand , the following complexes were also isolated : fac - ( ReBr ( CO ) ( 3 ) ( Hpyz ( B ) ) ) , the tetrameric complexes fac - ( Re ( pyz ( A ) ) ( CO ) ( 3 ) ) ( 4 ) and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ) ( 4 ) , and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ( H ( 2 ) O ) ) ( where Hpyz ( A ) and Hpyz ( B ) are pyrazolones derived by cyclization of H ( 2 ) L ( A ) and H ( 2 ) L ( B ) , respectively ) .
	manualset3
235321	15	421793	7	NULL	NULL	0	NULL	pyrazolones	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Besides the adducts fac - ( ReX ( CO ) ( 3 ) ( H ( 2 ) L ) ) , in which the rhenium is coordinated to three carbonyl groups , the X anion , and the N , S-bidentate thiosemicarbazone ligand , the following complexes were also isolated : fac - ( ReBr ( CO ) ( 3 ) ( Hpyz ( B ) ) ) , the tetrameric complexes fac - ( Re ( pyz ( A ) ) ( CO ) ( 3 ) ) ( 4 ) and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ) ( 4 ) , and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ( H ( 2 ) O ) ) ( where Hpyz ( A ) and Hpyz ( B ) are pyrazolones derived by cyclization of H ( 2 ) L ( A ) and H ( 2 ) L ( B ) , respectively ) .
	manualset3
235322	16	421793	7	NULL	NULL	0	NULL	cyclization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Besides the adducts fac - ( ReX ( CO ) ( 3 ) ( H ( 2 ) L ) ) , in which the rhenium is coordinated to three carbonyl groups , the X anion , and the N , S-bidentate thiosemicarbazone ligand , the following complexes were also isolated : fac - ( ReBr ( CO ) ( 3 ) ( Hpyz ( B ) ) ) , the tetrameric complexes fac - ( Re ( pyz ( A ) ) ( CO ) ( 3 ) ) ( 4 ) and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ) ( 4 ) , and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ( H ( 2 ) O ) ) ( where Hpyz ( A ) and Hpyz ( B ) are pyrazolones derived by cyclization of H ( 2 ) L ( A ) and H ( 2 ) L ( B ) , respectively ) .
	manualset3
235323	17	421793	7	NULL	NULL	0	NULL	H ( 2 ) L ( A )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Besides the adducts fac - ( ReX ( CO ) ( 3 ) ( H ( 2 ) L ) ) , in which the rhenium is coordinated to three carbonyl groups , the X anion , and the N , S-bidentate thiosemicarbazone ligand , the following complexes were also isolated : fac - ( ReBr ( CO ) ( 3 ) ( Hpyz ( B ) ) ) , the tetrameric complexes fac - ( Re ( pyz ( A ) ) ( CO ) ( 3 ) ) ( 4 ) and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ) ( 4 ) , and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ( H ( 2 ) O ) ) ( where Hpyz ( A ) and Hpyz ( B ) are pyrazolones derived by cyclization of H ( 2 ) L ( A ) and H ( 2 ) L ( B ) , respectively ) .
	manualset3
235324	18	421793	7	NULL	NULL	0	NULL	H ( 2 ) L ( B ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Besides the adducts fac - ( ReX ( CO ) ( 3 ) ( H ( 2 ) L ) ) , in which the rhenium is coordinated to three carbonyl groups , the X anion , and the N , S-bidentate thiosemicarbazone ligand , the following complexes were also isolated : fac - ( ReBr ( CO ) ( 3 ) ( Hpyz ( B ) ) ) , the tetrameric complexes fac - ( Re ( pyz ( A ) ) ( CO ) ( 3 ) ) ( 4 ) and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ) ( 4 ) , and fac - ( Re ( pyz ( B ) ) ( CO ) ( 3 ) ( H ( 2 ) O ) ) ( where Hpyz ( A ) and Hpyz ( B ) are pyrazolones derived by cyclization of H ( 2 ) L ( A ) and H ( 2 ) L ( B ) , respectively ) .
	manualset3
235325	1	421794	7	NULL	NULL	0	NULL	 1 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	About 1 % of the exogenous ( 1 - ( 14 ) C ) palmitic acid was incorporated into C ( 27 ) , C ( 29 ) , and C ( 31 ) n-alkanes , which were identified by combined gas-liquid chromatography and mass spectrometry as the major components of the hydrocarbons of V. faba flowers .
	manualset3
235326	2	421794	7	NULL	NULL	NULL	NULL	exogenous ( 1 - ( 14 ) C ) palmitic acid	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	About 1 % of the exogenous ( 1 - ( 14 ) C ) palmitic acid was incorporated into C ( 27 ) , C ( 29 ) , and C ( 31 ) n-alkanes , which were identified by combined gas-liquid chromatography and mass spectrometry as the major components of the hydrocarbons of V. faba flowers .
	manualset3
235327	3	421794	7	NULL	NULL	0	NULL	C ( 27 ) n-alkanes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	About 1 % of the exogenous ( 1 - ( 14 ) C ) palmitic acid was incorporated into C ( 27 ) , C ( 29 ) , and C ( 31 ) n-alkanes , which were identified by combined gas-liquid chromatography and mass spectrometry as the major components of the hydrocarbons of V. faba flowers .
	manualset3
235328	4	421794	7	NULL	NULL	0	NULL	 C ( 29 ) n-alkanes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	About 1 % of the exogenous ( 1 - ( 14 ) C ) palmitic acid was incorporated into C ( 27 ) , C ( 29 ) , and C ( 31 ) n-alkanes , which were identified by combined gas-liquid chromatography and mass spectrometry as the major components of the hydrocarbons of V. faba flowers .
	manualset3
235329	5	421794	7	NULL	NULL	0	NULL	C ( 31 ) n-alkanes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	About 1 % of the exogenous ( 1 - ( 14 ) C ) palmitic acid was incorporated into C ( 27 ) , C ( 29 ) , and C ( 31 ) n-alkanes , which were identified by combined gas-liquid chromatography and mass spectrometry as the major components of the hydrocarbons of V. faba flowers .
	manualset3
235330	6	421794	7	NULL	NULL	0	NULL	combined gas-liquid chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	About 1 % of the exogenous ( 1 - ( 14 ) C ) palmitic acid was incorporated into C ( 27 ) , C ( 29 ) , and C ( 31 ) n-alkanes , which were identified by combined gas-liquid chromatography and mass spectrometry as the major components of the hydrocarbons of V. faba flowers .
	manualset3
235331	7	421794	7	NULL	NULL	0	NULL	mass spectrometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	About 1 % of the exogenous ( 1 - ( 14 ) C ) palmitic acid was incorporated into C ( 27 ) , C ( 29 ) , and C ( 31 ) n-alkanes , which were identified by combined gas-liquid chromatography and mass spectrometry as the major components of the hydrocarbons of V. faba flowers .
	manualset3
235332	8	421794	7	NULL	NULL	0	NULL	major components	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	About 1 % of the exogenous ( 1 - ( 14 ) C ) palmitic acid was incorporated into C ( 27 ) , C ( 29 ) , and C ( 31 ) n-alkanes , which were identified by combined gas-liquid chromatography and mass spectrometry as the major components of the hydrocarbons of V. faba flowers .
	manualset3
235333	9	421794	7	NULL	NULL	0	NULL	hydrocarbons	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	About 1 % of the exogenous ( 1 - ( 14 ) C ) palmitic acid was incorporated into C ( 27 ) , C ( 29 ) , and C ( 31 ) n-alkanes , which were identified by combined gas-liquid chromatography and mass spectrometry as the major components of the hydrocarbons of V. faba flowers .
	manualset3
235334	10	421794	7	NULL	NULL	0	NULL	 V. faba flowers	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	About 1 % of the exogenous ( 1 - ( 14 ) C ) palmitic acid was incorporated into C ( 27 ) , C ( 29 ) , and C ( 31 ) n-alkanes , which were identified by combined gas-liquid chromatography and mass spectrometry as the major components of the hydrocarbons of V. faba flowers .
	manualset3
235335	1	421795	7	NULL	NULL	0	NULL	uptake	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The uptake of Cu2 + from chloride was higher and faster than that from nitrate .
	manualset3
235336	2	421795	7	NULL	NULL	0	NULL	Cu2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The uptake of Cu2 + from chloride was higher and faster than that from nitrate .
	manualset3
235337	3	421795	7	NULL	NULL	0	NULL	chloride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The uptake of Cu2 + from chloride was higher and faster than that from nitrate .
	manualset3
235338	4	421795	7	NULL	NULL	0	NULL	nitrate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The uptake of Cu2 + from chloride was higher and faster than that from nitrate .
	manualset3
235339	1	421796	7	NULL	NULL	0	NULL	Trp179	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Trp179 , Phe196 and Phe119 form an aromatic cluster at the entrance of the catalytic center .
	manualset3
235340	2	421796	7	NULL	NULL	0	NULL	Phe196	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Trp179 , Phe196 and Phe119 form an aromatic cluster at the entrance of the catalytic center .
	manualset3
235341	3	421796	7	NULL	NULL	0	NULL	Phe119	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Trp179 , Phe196 and Phe119 form an aromatic cluster at the entrance of the catalytic center .
	manualset3
235342	4	421796	7	NULL	NULL	0	NULL	aromatic cluster	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Trp179 , Phe196 and Phe119 form an aromatic cluster at the entrance of the catalytic center .
	manualset3
235343	5	421796	7	NULL	NULL	0	NULL	entrance	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Trp179 , Phe196 and Phe119 form an aromatic cluster at the entrance of the catalytic center .
	manualset3
235344	6	421796	7	NULL	NULL	0	NULL	catalytic center 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Trp179 , Phe196 and Phe119 form an aromatic cluster at the entrance of the catalytic center .
	manualset3
235345	1	421797	7	NULL	NULL	0	NULL	Angiotensin II infusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin II infusion reduced the expression and activity of AMP-activated protein kinase .
	manualset3
235346	2	421797	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin II infusion reduced the expression and activity of AMP-activated protein kinase .
	manualset3
235347	3	421797	7	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin II infusion reduced the expression and activity of AMP-activated protein kinase .
	manualset3
235348	4	421797	7	NULL	NULL	0	NULL	AMP-activated protein kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin II infusion reduced the expression and activity of AMP-activated protein kinase .
	manualset3
235349	1	421798	7	NULL	NULL	0	NULL	reproducible method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An automated , simple , and reproducible method based on isotope dilution headspace gas chromatography/mass spectrometry developed previously for the determination of benzene in soft drinks was further improved by adding sodium sulfate to samples , lowering the gas chromatography oven starting temperature to narrow benzene peak width , and increasing sample injection volume .
	manualset3
235350	2	421798	7	NULL	NULL	0	NULL	isotope dilution headspace gas chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An automated , simple , and reproducible method based on isotope dilution headspace gas chromatography/mass spectrometry developed previously for the determination of benzene in soft drinks was further improved by adding sodium sulfate to samples , lowering the gas chromatography oven starting temperature to narrow benzene peak width , and increasing sample injection volume .
	manualset3
235351	3	421798	7	NULL	NULL	0	NULL	mass spectrometry 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An automated , simple , and reproducible method based on isotope dilution headspace gas chromatography/mass spectrometry developed previously for the determination of benzene in soft drinks was further improved by adding sodium sulfate to samples , lowering the gas chromatography oven starting temperature to narrow benzene peak width , and increasing sample injection volume .
	manualset3
235352	4	421798	7	NULL	NULL	0	NULL	determination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An automated , simple , and reproducible method based on isotope dilution headspace gas chromatography/mass spectrometry developed previously for the determination of benzene in soft drinks was further improved by adding sodium sulfate to samples , lowering the gas chromatography oven starting temperature to narrow benzene peak width , and increasing sample injection volume .
	manualset3
235353	5	421798	7	NULL	NULL	0	NULL	benzene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An automated , simple , and reproducible method based on isotope dilution headspace gas chromatography/mass spectrometry developed previously for the determination of benzene in soft drinks was further improved by adding sodium sulfate to samples , lowering the gas chromatography oven starting temperature to narrow benzene peak width , and increasing sample injection volume .
	manualset3
235354	6	421798	7	NULL	NULL	0	NULL	soft drinks	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	An automated , simple , and reproducible method based on isotope dilution headspace gas chromatography/mass spectrometry developed previously for the determination of benzene in soft drinks was further improved by adding sodium sulfate to samples , lowering the gas chromatography oven starting temperature to narrow benzene peak width , and increasing sample injection volume .
	manualset3
235355	7	421798	7	NULL	NULL	0	NULL	sodium sulfate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An automated , simple , and reproducible method based on isotope dilution headspace gas chromatography/mass spectrometry developed previously for the determination of benzene in soft drinks was further improved by adding sodium sulfate to samples , lowering the gas chromatography oven starting temperature to narrow benzene peak width , and increasing sample injection volume .
	manualset3
235356	8	421798	7	NULL	NULL	NULL	NULL	samples	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An automated , simple , and reproducible method based on isotope dilution headspace gas chromatography/mass spectrometry developed previously for the determination of benzene in soft drinks was further improved by adding sodium sulfate to samples , lowering the gas chromatography oven starting temperature to narrow benzene peak width , and increasing sample injection volume .
	manualset3
235357	9	421798	7	NULL	NULL	NULL	NULL	gas chromatography oven	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An automated , simple , and reproducible method based on isotope dilution headspace gas chromatography/mass spectrometry developed previously for the determination of benzene in soft drinks was further improved by adding sodium sulfate to samples , lowering the gas chromatography oven starting temperature to narrow benzene peak width , and increasing sample injection volume .
	manualset3
235358	10	421798	7	NULL	NULL	0	NULL	temperature 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An automated , simple , and reproducible method based on isotope dilution headspace gas chromatography/mass spectrometry developed previously for the determination of benzene in soft drinks was further improved by adding sodium sulfate to samples , lowering the gas chromatography oven starting temperature to narrow benzene peak width , and increasing sample injection volume .
	manualset3
235359	11	421798	7	NULL	NULL	0	NULL	benzene peak width	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An automated , simple , and reproducible method based on isotope dilution headspace gas chromatography/mass spectrometry developed previously for the determination of benzene in soft drinks was further improved by adding sodium sulfate to samples , lowering the gas chromatography oven starting temperature to narrow benzene peak width , and increasing sample injection volume .
	manualset3
235360	12	421798	7	NULL	NULL	0	NULL	sample injection volume 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An automated , simple , and reproducible method based on isotope dilution headspace gas chromatography/mass spectrometry developed previously for the determination of benzene in soft drinks was further improved by adding sodium sulfate to samples , lowering the gas chromatography oven starting temperature to narrow benzene peak width , and increasing sample injection volume .
	manualset3
235361	1	421799	7	NULL	NULL	0	NULL	recent study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A recent study of Lee R Hagey characterized bile acid composition of over 600 species of vertebrates , showing that bile acid composition of bile has been the subject of an interesting evolutionary phenomenon and that it is a chemical marker of biodiversity in vertebrates .
	manualset3
235362	2	421799	7	NULL	NULL	0	NULL	Lee R Hagey	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A recent study of Lee R Hagey characterized bile acid composition of over 600 species of vertebrates , showing that bile acid composition of bile has been the subject of an interesting evolutionary phenomenon and that it is a chemical marker of biodiversity in vertebrates .
	manualset3
235363	3	421799	7	NULL	NULL	0	NULL	bile acid composition	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A recent study of Lee R Hagey characterized bile acid composition of over 600 species of vertebrates , showing that bile acid composition of bile has been the subject of an interesting evolutionary phenomenon and that it is a chemical marker of biodiversity in vertebrates .
	manualset3
235364	4	421799	7	NULL	NULL	0	NULL	 600 species 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A recent study of Lee R Hagey characterized bile acid composition of over 600 species of vertebrates , showing that bile acid composition of bile has been the subject of an interesting evolutionary phenomenon and that it is a chemical marker of biodiversity in vertebrates .
	manualset3
235365	5	421799	7	NULL	NULL	0	NULL	vertebrates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A recent study of Lee R Hagey characterized bile acid composition of over 600 species of vertebrates , showing that bile acid composition of bile has been the subject of an interesting evolutionary phenomenon and that it is a chemical marker of biodiversity in vertebrates .
	manualset3
235366	6	421799	7	NULL	NULL	0	NULL	bile acid composition	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A recent study of Lee R Hagey characterized bile acid composition of over 600 species of vertebrates , showing that bile acid composition of bile has been the subject of an interesting evolutionary phenomenon and that it is a chemical marker of biodiversity in vertebrates .
	manualset3
235367	7	421799	7	NULL	NULL	0	NULL	bile	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A recent study of Lee R Hagey characterized bile acid composition of over 600 species of vertebrates , showing that bile acid composition of bile has been the subject of an interesting evolutionary phenomenon and that it is a chemical marker of biodiversity in vertebrates .
	manualset3
235368	8	421799	7	NULL	NULL	0	NULL	subject 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A recent study of Lee R Hagey characterized bile acid composition of over 600 species of vertebrates , showing that bile acid composition of bile has been the subject of an interesting evolutionary phenomenon and that it is a chemical marker of biodiversity in vertebrates .
	manualset3
235369	9	421799	7	NULL	NULL	0	NULL	evolutionary phenomenon	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A recent study of Lee R Hagey characterized bile acid composition of over 600 species of vertebrates , showing that bile acid composition of bile has been the subject of an interesting evolutionary phenomenon and that it is a chemical marker of biodiversity in vertebrates .
	manualset3
235370	10	421799	7	NULL	NULL	0	NULL	chemical marker	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A recent study of Lee R Hagey characterized bile acid composition of over 600 species of vertebrates , showing that bile acid composition of bile has been the subject of an interesting evolutionary phenomenon and that it is a chemical marker of biodiversity in vertebrates .
	manualset3
235371	11	421799	7	NULL	NULL	0	NULL	biodiversity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A recent study of Lee R Hagey characterized bile acid composition of over 600 species of vertebrates , showing that bile acid composition of bile has been the subject of an interesting evolutionary phenomenon and that it is a chemical marker of biodiversity in vertebrates .
	manualset3
235372	12	421799	7	NULL	NULL	0	NULL	 vertebrates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A recent study of Lee R Hagey characterized bile acid composition of over 600 species of vertebrates , showing that bile acid composition of bile has been the subject of an interesting evolutionary phenomenon and that it is a chemical marker of biodiversity in vertebrates .
	manualset3
235373	1	421800	7	NULL	NULL	0	NULL	Mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations of the puroindoline genes , which are located on chromosome 5DS , control a majority of grain texture variations .
	manualset3
235374	2	421800	7	NULL	NULL	0	NULL	puroindoline genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations of the puroindoline genes , which are located on chromosome 5DS , control a majority of grain texture variations .
	manualset3
235375	3	421800	7	NULL	NULL	0	NULL	chromosome 5DS	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations of the puroindoline genes , which are located on chromosome 5DS , control a majority of grain texture variations .
	manualset3
235376	4	421800	7	NULL	NULL	0	NULL	majority 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations of the puroindoline genes , which are located on chromosome 5DS , control a majority of grain texture variations .
	manualset3
235377	5	421800	7	NULL	NULL	0	NULL	grain texture variations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutations of the puroindoline genes , which are located on chromosome 5DS , control a majority of grain texture variations .
	manualset3
235378	1	421801	7	NULL	NULL	0	NULL	survey	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey of 355 college students was carried out to determine the prevalence of the psychiatric disorder bulimia ( the binge-eating syndrome ) .
	manualset3
235379	2	421801	7	NULL	NULL	0	NULL	355 college students 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey of 355 college students was carried out to determine the prevalence of the psychiatric disorder bulimia ( the binge-eating syndrome ) .
	manualset3
235380	3	421801	7	NULL	NULL	0	NULL	prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey of 355 college students was carried out to determine the prevalence of the psychiatric disorder bulimia ( the binge-eating syndrome ) .
	manualset3
235381	4	421801	7	NULL	NULL	0	NULL	psychiatric disorder bulimia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey of 355 college students was carried out to determine the prevalence of the psychiatric disorder bulimia ( the binge-eating syndrome ) .
	manualset3
235382	5	421801	7	NULL	NULL	0	NULL	binge-eating syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	A survey of 355 college students was carried out to determine the prevalence of the psychiatric disorder bulimia ( the binge-eating syndrome ) .
	manualset3
235383	1	421802	7	NULL	NULL	0	NULL	introduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been found that the introduction of the novel 3-n-butylamino-2-hydroxypropyloxy moiety in place of the classical tert-beta-aminoethoxy group leads to enhancement of antifertility activity .
	manualset3
235384	2	421802	7	NULL	NULL	0	NULL	novel 3-n-butylamino-2-hydroxypropyloxy moiety	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been found that the introduction of the novel 3-n-butylamino-2-hydroxypropyloxy moiety in place of the classical tert-beta-aminoethoxy group leads to enhancement of antifertility activity .
	manualset3
235385	3	421802	7	NULL	NULL	0	NULL	classical tert-beta-aminoethoxy group	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been found that the introduction of the novel 3-n-butylamino-2-hydroxypropyloxy moiety in place of the classical tert-beta-aminoethoxy group leads to enhancement of antifertility activity .
	manualset3
235386	4	421802	7	NULL	NULL	0	NULL	antifertility activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It has been found that the introduction of the novel 3-n-butylamino-2-hydroxypropyloxy moiety in place of the classical tert-beta-aminoethoxy group leads to enhancement of antifertility activity .
	manualset3
235387	1	421803	7	NULL	NULL	0	NULL	Food	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	( Food and nutrition management in the Netherlands ; control of the results of social welfare .
	manualset3
235388	2	421803	7	NULL	NULL	0	NULL	nutrition management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Food and nutrition management in the Netherlands ; control of the results of social welfare .
	manualset3
235389	3	421803	7	NULL	NULL	0	NULL	Netherlands	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Food and nutrition management in the Netherlands ; control of the results of social welfare .
	manualset3
235390	4	421803	7	NULL	NULL	0	NULL	control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Food and nutrition management in the Netherlands ; control of the results of social welfare .
	manualset3
235391	5	421803	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Food and nutrition management in the Netherlands ; control of the results of social welfare .
	manualset3
235392	6	421803	7	NULL	NULL	0	NULL	social welfare	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	( Food and nutrition management in the Netherlands ; control of the results of social welfare .
	manualset3
235393	1	421804	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This led to a study of the effect of formamide on the melting temperature ( T ( m ) ) of double-stranded DNA in solution or bound to hydroxyapatite .
	manualset3
235394	2	421804	7	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This led to a study of the effect of formamide on the melting temperature ( T ( m ) ) of double-stranded DNA in solution or bound to hydroxyapatite .
	manualset3
235395	3	421804	7	NULL	NULL	0	NULL	formamide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This led to a study of the effect of formamide on the melting temperature ( T ( m ) ) of double-stranded DNA in solution or bound to hydroxyapatite .
	manualset3
235396	4	421804	7	NULL	NULL	0	NULL	melting temperature ( T ( m ) )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This led to a study of the effect of formamide on the melting temperature ( T ( m ) ) of double-stranded DNA in solution or bound to hydroxyapatite .
	manualset3
235397	5	421804	7	NULL	NULL	0	NULL	double-stranded DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	This led to a study of the effect of formamide on the melting temperature ( T ( m ) ) of double-stranded DNA in solution or bound to hydroxyapatite .
	manualset3
235398	6	421804	7	NULL	NULL	0	NULL	solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This led to a study of the effect of formamide on the melting temperature ( T ( m ) ) of double-stranded DNA in solution or bound to hydroxyapatite .
	manualset3
235399	7	421804	7	NULL	NULL	0	NULL	hydroxyapatite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This led to a study of the effect of formamide on the melting temperature ( T ( m ) ) of double-stranded DNA in solution or bound to hydroxyapatite .
	manualset3
235400	1	421805	7	NULL	NULL	0	NULL	cell types	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The cell types of the plant root are first specified early during embryogenesis and are maintained throughout plant life .
	manualset3
235401	2	421805	7	NULL	NULL	0	NULL	plant root	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The cell types of the plant root are first specified early during embryogenesis and are maintained throughout plant life .
	manualset3
235402	3	421805	7	NULL	NULL	0	NULL	embryogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cell types of the plant root are first specified early during embryogenesis and are maintained throughout plant life .
	manualset3
235403	4	421805	7	NULL	NULL	0	NULL	plant life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cell types of the plant root are first specified early during embryogenesis and are maintained throughout plant life .
	manualset3
235404	1	421806	7	NULL	NULL	0	NULL	Fractures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Fractures of the middle third of the face ) .
	manualset3
235405	2	421806	7	NULL	NULL	0	NULL	middle third 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Fractures of the middle third of the face ) .
	manualset3
235406	3	421806	7	NULL	NULL	0	NULL	face 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Fractures of the middle third of the face ) .
	manualset3
235407	1	421807	7	NULL	NULL	NULL	NULL	autopsy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An autopsy was performed and her skull was found to be thickened circumferentially .
	manualset3
235408	2	421807	7	NULL	NULL	0	NULL	skull 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An autopsy was performed and her skull was found to be thickened circumferentially .
	manualset3
235409	1	421808	7	NULL	NULL	0	NULL	 gene frequencies	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene frequencies were similar to those in other Spanish populations but the isolated valley of Arratia deviated significantly with increased frequencies of the M2 and M3 alleles and a decrease of the M1 allele .
	manualset3
235410	2	421808	7	NULL	NULL	0	NULL	Spanish populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene frequencies were similar to those in other Spanish populations but the isolated valley of Arratia deviated significantly with increased frequencies of the M2 and M3 alleles and a decrease of the M1 allele .
	manualset3
235411	3	421808	7	NULL	NULL	0	NULL	 isolated valley of Arratia	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene frequencies were similar to those in other Spanish populations but the isolated valley of Arratia deviated significantly with increased frequencies of the M2 and M3 alleles and a decrease of the M1 allele .
	manualset3
235412	4	421808	7	NULL	NULL	NULL	NULL	 increased frequencies	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The gene frequencies were similar to those in other Spanish populations but the isolated valley of Arratia deviated significantly with increased frequencies of the M2 and M3 alleles and a decrease of the M1 allele .
	manualset3
235413	5	421808	7	NULL	NULL	NULL	NULL	M2 alleles	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The gene frequencies were similar to those in other Spanish populations but the isolated valley of Arratia deviated significantly with increased frequencies of the M2 and M3 alleles and a decrease of the M1 allele .
	manualset3
235414	6	421808	7	NULL	NULL	0	NULL	M3 alleles	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene frequencies were similar to those in other Spanish populations but the isolated valley of Arratia deviated significantly with increased frequencies of the M2 and M3 alleles and a decrease of the M1 allele .
	manualset3
235415	7	421808	7	NULL	NULL	0	NULL	decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene frequencies were similar to those in other Spanish populations but the isolated valley of Arratia deviated significantly with increased frequencies of the M2 and M3 alleles and a decrease of the M1 allele .
	manualset3
235416	8	421808	7	NULL	NULL	0	NULL	M1 allele	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene frequencies were similar to those in other Spanish populations but the isolated valley of Arratia deviated significantly with increased frequencies of the M2 and M3 alleles and a decrease of the M1 allele .
	manualset3
235417	1	421809	7	NULL	NULL	0	NULL	Predictors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictors of flexibility and pain patterns in thoracolumbar and lumbar idiopathic scoliosis .
	manualset3
235418	2	421809	7	NULL	NULL	0	NULL	flexibility	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictors of flexibility and pain patterns in thoracolumbar and lumbar idiopathic scoliosis .
	manualset3
235419	3	421809	7	NULL	NULL	0	NULL	pain patterns	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictors of flexibility and pain patterns in thoracolumbar and lumbar idiopathic scoliosis .
	manualset3
235420	4	421809	7	NULL	NULL	0	NULL	thoracolumbar scoliosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictors of flexibility and pain patterns in thoracolumbar and lumbar idiopathic scoliosis .
	manualset3
235421	5	421809	7	NULL	NULL	0	NULL	lumbar idiopathic scoliosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Predictors of flexibility and pain patterns in thoracolumbar and lumbar idiopathic scoliosis .
	manualset3
235422	1	421810	7	NULL	NULL	0	NULL	Measurement 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of Stereopsis forms an important part of the clinical assessment of patients with disorders of ocular motility .
	manualset3
235423	2	421810	7	NULL	NULL	0	NULL	Stereopsis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of Stereopsis forms an important part of the clinical assessment of patients with disorders of ocular motility .
	manualset3
235424	3	421810	7	NULL	NULL	0	NULL	clinical assessment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of Stereopsis forms an important part of the clinical assessment of patients with disorders of ocular motility .
	manualset3
235425	4	421810	7	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of Stereopsis forms an important part of the clinical assessment of patients with disorders of ocular motility .
	manualset3
235426	5	421810	7	NULL	NULL	0	NULL	disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of Stereopsis forms an important part of the clinical assessment of patients with disorders of ocular motility .
	manualset3
235427	6	421810	7	NULL	NULL	0	NULL	ocular motility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurement of Stereopsis forms an important part of the clinical assessment of patients with disorders of ocular motility .
	manualset3
235428	1	421811	7	NULL	NULL	0	NULL	rhE2/E3BP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We also show that the rhE2/E3BP and bovine E2/E3BP cores bind E3s with a 2 : 1 stoichiometry , and propose that mammalian PDC comprises a heterogeneous population of assemblies incorporating a network of E3 ( and possibly E1 ) cross-bridges above the core surface .
	manualset3
235429	2	421811	7	NULL	NULL	0	NULL	bovine E2/E3BP cores	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We also show that the rhE2/E3BP and bovine E2/E3BP cores bind E3s with a 2 : 1 stoichiometry , and propose that mammalian PDC comprises a heterogeneous population of assemblies incorporating a network of E3 ( and possibly E1 ) cross-bridges above the core surface .
	manualset3
235430	3	421811	7	NULL	NULL	0	NULL	E3s	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We also show that the rhE2/E3BP and bovine E2/E3BP cores bind E3s with a 2 : 1 stoichiometry , and propose that mammalian PDC comprises a heterogeneous population of assemblies incorporating a network of E3 ( and possibly E1 ) cross-bridges above the core surface .
	manualset3
235431	4	421811	7	NULL	NULL	0	NULL	2 : 1 stoichiometry	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We also show that the rhE2/E3BP and bovine E2/E3BP cores bind E3s with a 2 : 1 stoichiometry , and propose that mammalian PDC comprises a heterogeneous population of assemblies incorporating a network of E3 ( and possibly E1 ) cross-bridges above the core surface .
	manualset3
235432	5	421811	7	NULL	NULL	0	NULL	mammalian PDC	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We also show that the rhE2/E3BP and bovine E2/E3BP cores bind E3s with a 2 : 1 stoichiometry , and propose that mammalian PDC comprises a heterogeneous population of assemblies incorporating a network of E3 ( and possibly E1 ) cross-bridges above the core surface .
	manualset3
235433	6	421811	7	NULL	NULL	0	NULL	heterogeneous population	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We also show that the rhE2/E3BP and bovine E2/E3BP cores bind E3s with a 2 : 1 stoichiometry , and propose that mammalian PDC comprises a heterogeneous population of assemblies incorporating a network of E3 ( and possibly E1 ) cross-bridges above the core surface .
	manualset3
235434	7	421811	7	NULL	NULL	NULL	NULL	assemblies 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We also show that the rhE2/E3BP and bovine E2/E3BP cores bind E3s with a 2 : 1 stoichiometry , and propose that mammalian PDC comprises a heterogeneous population of assemblies incorporating a network of E3 ( and possibly E1 ) cross-bridges above the core surface .
	manualset3
235435	8	421811	7	NULL	NULL	0	NULL	network	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We also show that the rhE2/E3BP and bovine E2/E3BP cores bind E3s with a 2 : 1 stoichiometry , and propose that mammalian PDC comprises a heterogeneous population of assemblies incorporating a network of E3 ( and possibly E1 ) cross-bridges above the core surface .
	manualset3
235436	9	421811	7	NULL	NULL	NULL	NULL	 E3 cross-bridges	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We also show that the rhE2/E3BP and bovine E2/E3BP cores bind E3s with a 2 : 1 stoichiometry , and propose that mammalian PDC comprises a heterogeneous population of assemblies incorporating a network of E3 ( and possibly E1 ) cross-bridges above the core surface .
	manualset3
235437	10	421811	7	NULL	NULL	0	NULL	E1	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We also show that the rhE2/E3BP and bovine E2/E3BP cores bind E3s with a 2 : 1 stoichiometry , and propose that mammalian PDC comprises a heterogeneous population of assemblies incorporating a network of E3 ( and possibly E1 ) cross-bridges above the core surface .
	manualset3
235438	11	421811	7	NULL	NULL	0	NULL	core surface	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	We also show that the rhE2/E3BP and bovine E2/E3BP cores bind E3s with a 2 : 1 stoichiometry , and propose that mammalian PDC comprises a heterogeneous population of assemblies incorporating a network of E3 ( and possibly E1 ) cross-bridges above the core surface .
	manualset3
235439	1	421812	7	NULL	NULL	0	NULL	 unexposed males	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	They were bred to unexposed males during TCDD exposure ( Experiment 1 ) and again after TCDD exposure ended ( Experiment 2 ) .
	manualset3
235440	2	421812	7	NULL	NULL	0	NULL	TCDD exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They were bred to unexposed males during TCDD exposure ( Experiment 1 ) and again after TCDD exposure ended ( Experiment 2 ) .
	manualset3
235441	3	421812	7	NULL	NULL	0	NULL	Experiment 1	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	They were bred to unexposed males during TCDD exposure ( Experiment 1 ) and again after TCDD exposure ended ( Experiment 2 ) .
	manualset3
235442	4	421812	7	NULL	NULL	0	NULL	TCDD exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	They were bred to unexposed males during TCDD exposure ( Experiment 1 ) and again after TCDD exposure ended ( Experiment 2 ) .
	manualset3
235443	5	421812	7	NULL	NULL	0	NULL	Experiment 2	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	They were bred to unexposed males during TCDD exposure ( Experiment 1 ) and again after TCDD exposure ended ( Experiment 2 ) .
	manualset3
235444	1	421813	7	NULL	NULL	0	NULL	Patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with breast cancer are unlikely to benefit from prophylactic irradiation of the contralateral breast .
	manualset3
235445	2	421813	7	NULL	NULL	0	NULL	breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with breast cancer are unlikely to benefit from prophylactic irradiation of the contralateral breast .
	manualset3
235446	3	421813	7	NULL	NULL	0	NULL	prophylactic irradiation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with breast cancer are unlikely to benefit from prophylactic irradiation of the contralateral breast .
	manualset3
235447	4	421813	7	NULL	NULL	0	NULL	contralateral breast 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Patients with breast cancer are unlikely to benefit from prophylactic irradiation of the contralateral breast .
	manualset3
235448	1	421814	7	NULL	NULL	0	NULL	PtdSer synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Both PtdSer synthesis and CD95-induced annexin V-FITC reactivity were abrogated in ATP-depleted cells .
	manualset3
235449	2	421814	7	NULL	NULL	0	NULL	CD95-induced annexin V-FITC reactivity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Both PtdSer synthesis and CD95-induced annexin V-FITC reactivity were abrogated in ATP-depleted cells .
	manualset3
235450	3	421814	7	NULL	NULL	0	NULL	ATP-depleted cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Both PtdSer synthesis and CD95-induced annexin V-FITC reactivity were abrogated in ATP-depleted cells .
	manualset3
235451	1	421815	7	NULL	NULL	0	NULL	process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter process includes formation of activating antibodies directed at the angiotensin ( Ang ) II receptor .
	manualset3
235452	2	421815	7	NULL	NULL	0	NULL	 formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter process includes formation of activating antibodies directed at the angiotensin ( Ang ) II receptor .
	manualset3
235453	3	421815	7	NULL	NULL	0	NULL	activating antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter process includes formation of activating antibodies directed at the angiotensin ( Ang ) II receptor .
	manualset3
235454	4	421815	7	NULL	NULL	0	NULL	angiotensin ( Ang ) II receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The latter process includes formation of activating antibodies directed at the angiotensin ( Ang ) II receptor .
	manualset3
235455	1	421816	7	NULL	NULL	0	NULL	autosomal dominant mode	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An autosomal dominant mode of inheritance would seem likely in both families .
	manualset3
235456	2	421816	7	NULL	NULL	0	NULL	inheritance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An autosomal dominant mode of inheritance would seem likely in both families .
	manualset3
235457	3	421816	7	NULL	NULL	0	NULL	families	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	An autosomal dominant mode of inheritance would seem likely in both families .
	manualset3
235458	1	421817	7	NULL	NULL	0	NULL	trichomonads	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When trichomonads were pre-treated with mAb to AP65 ( adhesin protein ) , or when trophozoites were separated from neutrophils using a Transwell chamber , neutrophil apoptosis was significantly reduced .
	manualset3
235459	2	421817	7	NULL	NULL	0	NULL	mAb	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	When trichomonads were pre-treated with mAb to AP65 ( adhesin protein ) , or when trophozoites were separated from neutrophils using a Transwell chamber , neutrophil apoptosis was significantly reduced .
	manualset3
235460	3	421817	7	NULL	NULL	0	NULL	AP65 ( adhesin protein )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	When trichomonads were pre-treated with mAb to AP65 ( adhesin protein ) , or when trophozoites were separated from neutrophils using a Transwell chamber , neutrophil apoptosis was significantly reduced .
	manualset3
235461	4	421817	7	NULL	NULL	0	NULL	trophozoites	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When trichomonads were pre-treated with mAb to AP65 ( adhesin protein ) , or when trophozoites were separated from neutrophils using a Transwell chamber , neutrophil apoptosis was significantly reduced .
	manualset3
235462	5	421817	7	NULL	NULL	0	NULL	neutrophils	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	When trichomonads were pre-treated with mAb to AP65 ( adhesin protein ) , or when trophozoites were separated from neutrophils using a Transwell chamber , neutrophil apoptosis was significantly reduced .
	manualset3
235463	6	421817	7	NULL	NULL	0	NULL	Transwell chamber	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	When trichomonads were pre-treated with mAb to AP65 ( adhesin protein ) , or when trophozoites were separated from neutrophils using a Transwell chamber , neutrophil apoptosis was significantly reduced .
	manualset3
235464	7	421817	7	NULL	NULL	0	NULL	neutrophil apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When trichomonads were pre-treated with mAb to AP65 ( adhesin protein ) , or when trophozoites were separated from neutrophils using a Transwell chamber , neutrophil apoptosis was significantly reduced .
	manualset3
235465	1	421818	7	NULL	NULL	0	NULL	 cardinal findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cardinal findings in brain death are coma , absence of brainstem reflexes , and apnea .
	manualset3
235466	2	421818	7	NULL	NULL	0	NULL	brain death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cardinal findings in brain death are coma , absence of brainstem reflexes , and apnea .
	manualset3
235467	3	421818	7	NULL	NULL	0	NULL	 coma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cardinal findings in brain death are coma , absence of brainstem reflexes , and apnea .
	manualset3
235468	4	421818	7	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cardinal findings in brain death are coma , absence of brainstem reflexes , and apnea .
	manualset3
235469	5	421818	7	NULL	NULL	0	NULL	brainstem reflexes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cardinal findings in brain death are coma , absence of brainstem reflexes , and apnea .
	manualset3
235470	6	421818	7	NULL	NULL	0	NULL	apnea	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The cardinal findings in brain death are coma , absence of brainstem reflexes , and apnea .
	manualset3
235471	1	421819	7	NULL	NULL	0	NULL	Descending 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Descending quasi-axial projection of the disk during discography .
	manualset3
235472	2	421819	7	NULL	NULL	0	NULL	quasi-axial projection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Descending quasi-axial projection of the disk during discography .
	manualset3
235473	3	421819	7	NULL	NULL	0	NULL	 disk 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Descending quasi-axial projection of the disk during discography .
	manualset3
235474	4	421819	7	NULL	NULL	0	NULL	discography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Descending quasi-axial projection of the disk during discography .
	manualset3
235475	1	421820	7	NULL	NULL	0	NULL	 developed countries	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In developed countries S. pneumoniae probably accounts for 25 to 30 % of cases of pediatric community-acquired pneumonia .
	manualset3
235476	2	421820	7	NULL	NULL	0	NULL	S. pneumoniae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In developed countries S. pneumoniae probably accounts for 25 to 30 % of cases of pediatric community-acquired pneumonia .
	manualset3
235477	3	421820	7	NULL	NULL	0	NULL	25%	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In developed countries S. pneumoniae probably accounts for 25 to 30 % of cases of pediatric community-acquired pneumonia .
	manualset3
235478	4	421820	7	NULL	NULL	0	NULL	30 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In developed countries S. pneumoniae probably accounts for 25 to 30 % of cases of pediatric community-acquired pneumonia .
	manualset3
235479	5	421820	7	NULL	NULL	0	NULL	 cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In developed countries S. pneumoniae probably accounts for 25 to 30 % of cases of pediatric community-acquired pneumonia .
	manualset3
235480	6	421820	7	NULL	NULL	0	NULL	 pediatric community-acquired pneumonia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	In developed countries S. pneumoniae probably accounts for 25 to 30 % of cases of pediatric community-acquired pneumonia .
	manualset3
235662	1	421821	7	NULL	NULL	0	NULL	KU-9 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The KU-9 cells showed chromosome numbers ranging from 56 to 61 with consistent structural abnormalities being add ( 2 ) ( q31 ) , + add ( 11 ) ( p11 .2 ) , + add ( 13 ) ( p11 .1 ) , and + del ( 22 ) ( q12 ) .
	manualset3
235663	2	421821	7	NULL	NULL	0	NULL	chromosome numbers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The KU-9 cells showed chromosome numbers ranging from 56 to 61 with consistent structural abnormalities being add ( 2 ) ( q31 ) , + add ( 11 ) ( p11 .2 ) , + add ( 13 ) ( p11 .1 ) , and + del ( 22 ) ( q12 ) .
	manualset3
235664	3	421821	7	NULL	NULL	0	NULL	56 to 61 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The KU-9 cells showed chromosome numbers ranging from 56 to 61 with consistent structural abnormalities being add ( 2 ) ( q31 ) , + add ( 11 ) ( p11 .2 ) , + add ( 13 ) ( p11 .1 ) , and + del ( 22 ) ( q12 ) .
	manualset3
235665	4	421821	7	NULL	NULL	0	NULL	consistent structural abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The KU-9 cells showed chromosome numbers ranging from 56 to 61 with consistent structural abnormalities being add ( 2 ) ( q31 ) , + add ( 11 ) ( p11 .2 ) , + add ( 13 ) ( p11 .1 ) , and + del ( 22 ) ( q12 ) .
	manualset3
235666	5	421821	7	NULL	NULL	0	NULL	 add ( 2 ) ( q31 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The KU-9 cells showed chromosome numbers ranging from 56 to 61 with consistent structural abnormalities being add ( 2 ) ( q31 ) , + add ( 11 ) ( p11 .2 ) , + add ( 13 ) ( p11 .1 ) , and + del ( 22 ) ( q12 ) .
	manualset3
235667	6	421821	7	NULL	NULL	0	NULL	add ( 11 ) ( p11 .2 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The KU-9 cells showed chromosome numbers ranging from 56 to 61 with consistent structural abnormalities being add ( 2 ) ( q31 ) , + add ( 11 ) ( p11 .2 ) , + add ( 13 ) ( p11 .1 ) , and + del ( 22 ) ( q12 ) .
	manualset3
235668	7	421821	7	NULL	NULL	0	NULL	add ( 13 ) ( p11 .1 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The KU-9 cells showed chromosome numbers ranging from 56 to 61 with consistent structural abnormalities being add ( 2 ) ( q31 ) , + add ( 11 ) ( p11 .2 ) , + add ( 13 ) ( p11 .1 ) , and + del ( 22 ) ( q12 ) .
	manualset3
235669	8	421821	7	NULL	NULL	0	NULL	del ( 22 ) ( q12 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The KU-9 cells showed chromosome numbers ranging from 56 to 61 with consistent structural abnormalities being add ( 2 ) ( q31 ) , + add ( 11 ) ( p11 .2 ) , + add ( 13 ) ( p11 .1 ) , and + del ( 22 ) ( q12 ) .
	manualset3
235670	1	421822	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	There were pronounced effects of suspension on DNA concentration and on protein/DNA , which suggests that muscle atrophy was accompanied by a reduction in muscle cell size .
	manualset3
235671	2	421822	7	NULL	NULL	NULL	NULL	suspension 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There were pronounced effects of suspension on DNA concentration and on protein/DNA , which suggests that muscle atrophy was accompanied by a reduction in muscle cell size .
	manualset3
235672	3	421822	7	NULL	NULL	0	NULL	protein/DNA	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	There were pronounced effects of suspension on DNA concentration and on protein/DNA , which suggests that muscle atrophy was accompanied by a reduction in muscle cell size .
	manualset3
235673	4	421822	7	NULL	NULL	0	NULL	muscle atrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were pronounced effects of suspension on DNA concentration and on protein/DNA , which suggests that muscle atrophy was accompanied by a reduction in muscle cell size .
	manualset3
235674	5	421822	7	NULL	NULL	0	NULL	reduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There were pronounced effects of suspension on DNA concentration and on protein/DNA , which suggests that muscle atrophy was accompanied by a reduction in muscle cell size .
	manualset3
235675	6	421822	7	NULL	NULL	0	NULL	muscle cell size 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were pronounced effects of suspension on DNA concentration and on protein/DNA , which suggests that muscle atrophy was accompanied by a reduction in muscle cell size .
	manualset3
235676	7	421822	7	NULL	NULL	0	NULL	DNA concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There were pronounced effects of suspension on DNA concentration and on protein/DNA , which suggests that muscle atrophy was accompanied by a reduction in muscle cell size .
	manualset3
235677	1	421823	7	NULL	NULL	0	NULL	Transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Transplantation of Flk-1 + human bone marrow-derived mesenchymal stem cells promotes angiogenesis and neurogenesis after cerebral ischemia in rats .
	manualset3
235678	2	421823	7	NULL	NULL	0	NULL	 Flk-1 + human bone marrow-derived mesenchymal stem cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Transplantation of Flk-1 + human bone marrow-derived mesenchymal stem cells promotes angiogenesis and neurogenesis after cerebral ischemia in rats .
	manualset3
235679	3	421823	7	NULL	NULL	0	NULL	angiogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transplantation of Flk-1 + human bone marrow-derived mesenchymal stem cells promotes angiogenesis and neurogenesis after cerebral ischemia in rats .
	manualset3
235680	4	421823	7	NULL	NULL	0	NULL	neurogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Transplantation of Flk-1 + human bone marrow-derived mesenchymal stem cells promotes angiogenesis and neurogenesis after cerebral ischemia in rats .
	manualset3
235681	5	421823	7	NULL	NULL	0	NULL	cerebral ischemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Transplantation of Flk-1 + human bone marrow-derived mesenchymal stem cells promotes angiogenesis and neurogenesis after cerebral ischemia in rats .
	manualset3
235682	6	421823	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Transplantation of Flk-1 + human bone marrow-derived mesenchymal stem cells promotes angiogenesis and neurogenesis after cerebral ischemia in rats .
	manualset3
235683	1	421824	7	NULL	NULL	0	NULL	Immunoprecipitation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation from transfected HEK293 cells revealed co-precipitation of native p22phox with yfp-tagged Nox1 , Nox2 , and Nox4 .
	manualset3
235684	2	421824	7	NULL	NULL	0	NULL	transfected HEK293 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation from transfected HEK293 cells revealed co-precipitation of native p22phox with yfp-tagged Nox1 , Nox2 , and Nox4 .
	manualset3
235685	3	421824	7	NULL	NULL	0	NULL	co-precipitation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation from transfected HEK293 cells revealed co-precipitation of native p22phox with yfp-tagged Nox1 , Nox2 , and Nox4 .
	manualset3
235686	4	421824	7	NULL	NULL	0	NULL	native p22phox	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation from transfected HEK293 cells revealed co-precipitation of native p22phox with yfp-tagged Nox1 , Nox2 , and Nox4 .
	manualset3
235687	5	421824	7	NULL	NULL	0	NULL	yfp-tagged Nox1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation from transfected HEK293 cells revealed co-precipitation of native p22phox with yfp-tagged Nox1 , Nox2 , and Nox4 .
	manualset3
235688	6	421824	7	NULL	NULL	0	NULL	Nox2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation from transfected HEK293 cells revealed co-precipitation of native p22phox with yfp-tagged Nox1 , Nox2 , and Nox4 .
	manualset3
235689	7	421824	7	NULL	NULL	0	NULL	Nox4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Immunoprecipitation from transfected HEK293 cells revealed co-precipitation of native p22phox with yfp-tagged Nox1 , Nox2 , and Nox4 .
	manualset3
235690	1	421825	7	NULL	NULL	0	NULL	 surface structure 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The surface structure of Cu ( 100 ) modified by chloride and iodide has been studied in an electrochemical environment by means of in-situ scanning tunneling microscopy in combination with in-situ surface X-ray diffraction with a particular focus on adsorbate and potential dependent surface relaxation phenomena .
	manualset3
235691	2	421825	7	NULL	NULL	0	NULL	Cu ( 100 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The surface structure of Cu ( 100 ) modified by chloride and iodide has been studied in an electrochemical environment by means of in-situ scanning tunneling microscopy in combination with in-situ surface X-ray diffraction with a particular focus on adsorbate and potential dependent surface relaxation phenomena .
	manualset3
235692	3	421825	7	NULL	NULL	0	NULL	chloride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The surface structure of Cu ( 100 ) modified by chloride and iodide has been studied in an electrochemical environment by means of in-situ scanning tunneling microscopy in combination with in-situ surface X-ray diffraction with a particular focus on adsorbate and potential dependent surface relaxation phenomena .
	manualset3
235693	4	421825	7	NULL	NULL	0	NULL	iodide 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The surface structure of Cu ( 100 ) modified by chloride and iodide has been studied in an electrochemical environment by means of in-situ scanning tunneling microscopy in combination with in-situ surface X-ray diffraction with a particular focus on adsorbate and potential dependent surface relaxation phenomena .
	manualset3
235694	5	421825	7	NULL	NULL	0	NULL	electrochemical environment 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The surface structure of Cu ( 100 ) modified by chloride and iodide has been studied in an electrochemical environment by means of in-situ scanning tunneling microscopy in combination with in-situ surface X-ray diffraction with a particular focus on adsorbate and potential dependent surface relaxation phenomena .
	manualset3
235695	6	421825	7	NULL	NULL	0	NULL	in-situ scanning tunneling microscopy 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The surface structure of Cu ( 100 ) modified by chloride and iodide has been studied in an electrochemical environment by means of in-situ scanning tunneling microscopy in combination with in-situ surface X-ray diffraction with a particular focus on adsorbate and potential dependent surface relaxation phenomena .
	manualset3
235696	7	421825	7	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The surface structure of Cu ( 100 ) modified by chloride and iodide has been studied in an electrochemical environment by means of in-situ scanning tunneling microscopy in combination with in-situ surface X-ray diffraction with a particular focus on adsorbate and potential dependent surface relaxation phenomena .
	manualset3
235697	8	421825	7	NULL	NULL	0	NULL	in-situ surface X-ray diffraction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The surface structure of Cu ( 100 ) modified by chloride and iodide has been studied in an electrochemical environment by means of in-situ scanning tunneling microscopy in combination with in-situ surface X-ray diffraction with a particular focus on adsorbate and potential dependent surface relaxation phenomena .
	manualset3
235698	9	421825	7	NULL	NULL	0	NULL	focus 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The surface structure of Cu ( 100 ) modified by chloride and iodide has been studied in an electrochemical environment by means of in-situ scanning tunneling microscopy in combination with in-situ surface X-ray diffraction with a particular focus on adsorbate and potential dependent surface relaxation phenomena .
	manualset3
235699	10	421825	7	NULL	NULL	0	NULL	adsorbate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The surface structure of Cu ( 100 ) modified by chloride and iodide has been studied in an electrochemical environment by means of in-situ scanning tunneling microscopy in combination with in-situ surface X-ray diffraction with a particular focus on adsorbate and potential dependent surface relaxation phenomena .
	manualset3
235700	11	421825	7	NULL	NULL	0	NULL	potential dependent surface relaxation phenomena	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The surface structure of Cu ( 100 ) modified by chloride and iodide has been studied in an electrochemical environment by means of in-situ scanning tunneling microscopy in combination with in-situ surface X-ray diffraction with a particular focus on adsorbate and potential dependent surface relaxation phenomena .
	manualset3
235701	1	421826	7	NULL	NULL	0	NULL	Allogeneic hematopoietic stem cell transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Allogeneic hematopoietic stem cell transplantation in children with sickle cell disease .
	manualset3
235702	2	421826	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Allogeneic hematopoietic stem cell transplantation in children with sickle cell disease .
	manualset3
235703	3	421826	7	NULL	NULL	0	NULL	sickle cell disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Allogeneic hematopoietic stem cell transplantation in children with sickle cell disease .
	manualset3
235704	1	421827	7	NULL	NULL	0	NULL	Embryotropic action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Embryotropic action of the triazine herbicide polyzin 50 ) .
	manualset3
235707	2	421827	7	NULL	NULL	0	NULL	triazine herbicide polyzin 50	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Embryotropic action of the triazine herbicide polyzin 50 ) .
	manualset3
235710	1	421828	7	NULL	NULL	NULL	NULL	average	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An average of 2.5 days elapses between RU 486 intake and the onset of uterine bleeding .
	manualset3
235711	2	421828	7	NULL	NULL	0	NULL	2.5 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	An average of 2.5 days elapses between RU 486 intake and the onset of uterine bleeding .
	manualset3
235712	3	421828	7	NULL	NULL	0	NULL	RU 486 intake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An average of 2.5 days elapses between RU 486 intake and the onset of uterine bleeding .
	manualset3
235713	4	421828	7	NULL	NULL	0	NULL	onset	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An average of 2.5 days elapses between RU 486 intake and the onset of uterine bleeding .
	manualset3
235714	5	421828	7	NULL	NULL	0	NULL	uterine bleeding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An average of 2.5 days elapses between RU 486 intake and the onset of uterine bleeding .
	manualset3
235715	1	421829	7	NULL	NULL	0	NULL	p less than 0.05 ) 4	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( p less than 0.05 ) 4 ) Placental implantation site had no relation with labor duration , fetal weight , placental weight , amount of hemorrhage during labor and cord-coiling .
	manualset3
235716	2	421829	7	NULL	NULL	0	NULL	Placental implantation site 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( p less than 0.05 ) 4 ) Placental implantation site had no relation with labor duration , fetal weight , placental weight , amount of hemorrhage during labor and cord-coiling .
	manualset3
235717	3	421829	7	NULL	NULL	0	NULL	no relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	( p less than 0.05 ) 4 ) Placental implantation site had no relation with labor duration , fetal weight , placental weight , amount of hemorrhage during labor and cord-coiling .
	manualset3
235718	4	421829	7	NULL	NULL	0	NULL	labor duration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( p less than 0.05 ) 4 ) Placental implantation site had no relation with labor duration , fetal weight , placental weight , amount of hemorrhage during labor and cord-coiling .
	manualset3
235719	5	421829	7	NULL	NULL	0	NULL	fetal weight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( p less than 0.05 ) 4 ) Placental implantation site had no relation with labor duration , fetal weight , placental weight , amount of hemorrhage during labor and cord-coiling .
	manualset3
235720	6	421829	7	NULL	NULL	0	NULL	placental weight 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( p less than 0.05 ) 4 ) Placental implantation site had no relation with labor duration , fetal weight , placental weight , amount of hemorrhage during labor and cord-coiling .
	manualset3
235721	7	421829	7	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( p less than 0.05 ) 4 ) Placental implantation site had no relation with labor duration , fetal weight , placental weight , amount of hemorrhage during labor and cord-coiling .
	manualset3
235722	8	421829	7	NULL	NULL	0	NULL	hemorrhage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( p less than 0.05 ) 4 ) Placental implantation site had no relation with labor duration , fetal weight , placental weight , amount of hemorrhage during labor and cord-coiling .
	manualset3
235723	9	421829	7	NULL	NULL	NULL	NULL	labor	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( p less than 0.05 ) 4 ) Placental implantation site had no relation with labor duration , fetal weight , placental weight , amount of hemorrhage during labor and cord-coiling .
	manualset3
235724	10	421829	7	NULL	NULL	0	NULL	cord-coiling	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( p less than 0.05 ) 4 ) Placental implantation site had no relation with labor duration , fetal weight , placental weight , amount of hemorrhage during labor and cord-coiling .
	manualset3
235725	1	421830	7	NULL	NULL	0	NULL	decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It was not associated with a decrease in insulin receptor autophosphorylation .
	manualset3
235726	2	421830	7	NULL	NULL	0	NULL	insulin receptor autophosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It was not associated with a decrease in insulin receptor autophosphorylation .
	manualset3
235727	1	421831	7	NULL	NULL	0	NULL	Reality therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Reality therapy : a realistic approach to enterostomy rehabilitation .
	manualset3
235728	2	421831	7	NULL	NULL	0	NULL	realistic approach 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reality therapy : a realistic approach to enterostomy rehabilitation .
	manualset3
235729	3	421831	7	NULL	NULL	0	NULL	enterostomy rehabilitation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Reality therapy : a realistic approach to enterostomy rehabilitation .
	manualset3
235730	1	421832	7	NULL	NULL	0	NULL	Persistent symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Persistent symptoms were usually related to arrhythmias .
	manualset3
235731	2	421832	7	NULL	NULL	0	NULL	arrhythmias	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Persistent symptoms were usually related to arrhythmias .
	manualset3
235732	1	421833	7	NULL	NULL	0	NULL	Local interferon-production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Local interferon-production in the respiratory - and genital tract following infection with rhinotracheitis ( IBR ) and herpes exanthema ( IPV ) virus ) .
	manualset3
235733	2	421833	7	NULL	NULL	0	NULL	respiratory - tract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Local interferon-production in the respiratory - and genital tract following infection with rhinotracheitis ( IBR ) and herpes exanthema ( IPV ) virus ) .
	manualset3
235734	3	421833	7	NULL	NULL	0	NULL	genital tract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Local interferon-production in the respiratory - and genital tract following infection with rhinotracheitis ( IBR ) and herpes exanthema ( IPV ) virus ) .
	manualset3
235735	4	421833	7	NULL	NULL	0	NULL	 infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Local interferon-production in the respiratory - and genital tract following infection with rhinotracheitis ( IBR ) and herpes exanthema ( IPV ) virus ) .
	manualset3
235736	5	421833	7	NULL	NULL	0	NULL	rhinotracheitis ( IBR ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Local interferon-production in the respiratory - and genital tract following infection with rhinotracheitis ( IBR ) and herpes exanthema ( IPV ) virus ) .
	manualset3
235737	6	421833	7	NULL	NULL	0	NULL	herpes exanthema ( IPV ) virus )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Local interferon-production in the respiratory - and genital tract following infection with rhinotracheitis ( IBR ) and herpes exanthema ( IPV ) virus ) .
	manualset3
235738	1	421834	7	NULL	NULL	0	NULL	 development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of transfer of response to patterning by monkeys .
	manualset3
235739	2	421834	7	NULL	NULL	0	NULL	transfer	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of transfer of response to patterning by monkeys .
	manualset3
235740	3	421834	7	NULL	NULL	0	NULL	 response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of transfer of response to patterning by monkeys .
	manualset3
235741	4	421834	7	NULL	NULL	0	NULL	 patterning	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of transfer of response to patterning by monkeys .
	manualset3
235742	5	421834	7	NULL	NULL	0	NULL	monkeys	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The development of transfer of response to patterning by monkeys .
	manualset3
235743	1	421835	7	NULL	NULL	0	NULL	Diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Diagnosis and therapy of superficial tumors of the urinary bladder ) .
	manualset3
235744	2	421835	7	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Diagnosis and therapy of superficial tumors of the urinary bladder ) .
	manualset3
235745	3	421835	7	NULL	NULL	0	NULL	superficial tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Diagnosis and therapy of superficial tumors of the urinary bladder ) .
	manualset3
235746	4	421835	7	NULL	NULL	0	NULL	urinary bladder	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Diagnosis and therapy of superficial tumors of the urinary bladder ) .
	manualset3
237029	1	421836	7	NULL	NULL	0	NULL	axial length 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An axial length ) 25 mm was associated with the development of retinal tears ( p & lt ; 0.05 , Fisher 's exact test ) .
	manualset3
237030	2	421836	7	NULL	NULL	0	NULL	25 mm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	An axial length ) 25 mm was associated with the development of retinal tears ( p & lt ; 0.05 , Fisher 's exact test ) .
	manualset3
237031	3	421836	7	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An axial length ) 25 mm was associated with the development of retinal tears ( p & lt ; 0.05 , Fisher 's exact test ) .
	manualset3
237032	4	421836	7	NULL	NULL	0	NULL	retinal tears	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An axial length ) 25 mm was associated with the development of retinal tears ( p & lt ; 0.05 , Fisher 's exact test ) .
	manualset3
237035	5	421836	7	NULL	NULL	0	NULL	p & lt ; 0.05	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An axial length ) 25 mm was associated with the development of retinal tears ( p & lt ; 0.05 , Fisher 's exact test ) .
	manualset3
237036	6	421836	7	NULL	NULL	0	NULL	Fisher 's exact test	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An axial length ) 25 mm was associated with the development of retinal tears ( p & lt ; 0.05 , Fisher 's exact test ) .
	manualset3
237039	1	421837	7	NULL	NULL	0	NULL	agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The different responsiveness to agents activating PKA - and PKC-dependent pathways may depend on the cellular state of differentiation , or alternatively , cancer cell line-specific defects .
	manualset3
237040	2	421837	7	NULL	NULL	0	NULL	PKA - dependent pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The different responsiveness to agents activating PKA - and PKC-dependent pathways may depend on the cellular state of differentiation , or alternatively , cancer cell line-specific defects .
	manualset3
237041	3	421837	7	NULL	NULL	0	NULL	PKC-dependent pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The different responsiveness to agents activating PKA - and PKC-dependent pathways may depend on the cellular state of differentiation , or alternatively , cancer cell line-specific defects .
	manualset3
237042	4	421837	7	NULL	NULL	0	NULL	cellular state	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The different responsiveness to agents activating PKA - and PKC-dependent pathways may depend on the cellular state of differentiation , or alternatively , cancer cell line-specific defects .
	manualset3
237043	5	421837	7	NULL	NULL	0	NULL	 differentiation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The different responsiveness to agents activating PKA - and PKC-dependent pathways may depend on the cellular state of differentiation , or alternatively , cancer cell line-specific defects .
	manualset3
237044	6	421837	7	NULL	NULL	0	NULL	cancer cell line-specific defects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The different responsiveness to agents activating PKA - and PKC-dependent pathways may depend on the cellular state of differentiation , or alternatively , cancer cell line-specific defects .
	manualset3
237046	1	421838	7	NULL	NULL	0	NULL	Radical Resections	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Radical Resections of Advanced Intra-abdominal Cancer : Summary of Results in 100 Patients .
	manualset3
237047	2	421838	7	NULL	NULL	0	NULL	Advanced Intra-abdominal Cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Radical Resections of Advanced Intra-abdominal Cancer : Summary of Results in 100 Patients .
	manualset3
237048	3	421838	7	NULL	NULL	0	NULL	Summary	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Radical Resections of Advanced Intra-abdominal Cancer : Summary of Results in 100 Patients .
	manualset3
237050	4	421838	7	NULL	NULL	0	NULL	Results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Radical Resections of Advanced Intra-abdominal Cancer : Summary of Results in 100 Patients .
	manualset3
237052	5	421838	7	NULL	NULL	0	NULL	100 Patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Radical Resections of Advanced Intra-abdominal Cancer : Summary of Results in 100 Patients .
	manualset3
237055	1	421839	7	NULL	NULL	0	NULL	119 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 119 patients referred for barium pharyngography , both single - and double-contrast examinations were performed .
	manualset3
237056	2	421839	7	NULL	NULL	0	NULL	barium pharyngography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 119 patients referred for barium pharyngography , both single - and double-contrast examinations were performed .
	manualset3
237058	3	421839	7	NULL	NULL	0	NULL	single - contrast examinations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 119 patients referred for barium pharyngography , both single - and double-contrast examinations were performed .
	manualset3
237059	4	421839	7	NULL	NULL	0	NULL	double-contrast examinations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	In 119 patients referred for barium pharyngography , both single - and double-contrast examinations were performed .
	manualset3
237256	1	421840	7	NULL	NULL	0	NULL	Muscimol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscimol failed to produce hyperactivity , however , when injected into rats who had previously received an electrolytic median raphe lesion .
	manualset3
237257	2	421840	7	NULL	NULL	0	NULL	 hyperactivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscimol failed to produce hyperactivity , however , when injected into rats who had previously received an electrolytic median raphe lesion .
	manualset3
237258	3	421840	7	NULL	NULL	0	NULL	 rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscimol failed to produce hyperactivity , however , when injected into rats who had previously received an electrolytic median raphe lesion .
	manualset3
237259	4	421840	7	NULL	NULL	0	NULL	electrolytic median raphe lesion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Muscimol failed to produce hyperactivity , however , when injected into rats who had previously received an electrolytic median raphe lesion .
	manualset3
237260	1	421841	7	NULL	NULL	NULL	NULL	Reverse transcription-polymerase chain reaction	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Reverse transcription-polymerase chain reaction showed that TWIK-1 mRNA is present in the vestibular end organs , vestibular ganglion and cochlea .
	manualset3
237261	2	421841	7	NULL	NULL	0	NULL	TWIK-1 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Reverse transcription-polymerase chain reaction showed that TWIK-1 mRNA is present in the vestibular end organs , vestibular ganglion and cochlea .
	manualset3
237262	3	421841	7	NULL	NULL	0	NULL	vestibular end organs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Reverse transcription-polymerase chain reaction showed that TWIK-1 mRNA is present in the vestibular end organs , vestibular ganglion and cochlea .
	manualset3
237263	4	421841	7	NULL	NULL	NULL	NULL	vestibular  ganglion	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Reverse transcription-polymerase chain reaction showed that TWIK-1 mRNA is present in the vestibular end organs , vestibular ganglion and cochlea .
	manualset3
237264	5	421841	7	NULL	NULL	0	NULL	cochlea	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Reverse transcription-polymerase chain reaction showed that TWIK-1 mRNA is present in the vestibular end organs , vestibular ganglion and cochlea .
	manualset3
237265	1	421842	7	NULL	NULL	0	NULL	Effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of postmortem storage temperature on sea bass ( Dicentrarchus labrax ) muscle protein degradation : analysis by 2-D DIGE and MS .
	manualset3
237266	2	421842	7	NULL	NULL	0	NULL	postmortem storage temperature	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of postmortem storage temperature on sea bass ( Dicentrarchus labrax ) muscle protein degradation : analysis by 2-D DIGE and MS .
	manualset3
237267	3	421842	7	NULL	NULL	0	NULL	sea bass ( Dicentrarchus labrax )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of postmortem storage temperature on sea bass ( Dicentrarchus labrax ) muscle protein degradation : analysis by 2-D DIGE and MS .
	manualset3
237268	4	421842	7	NULL	NULL	0	NULL	muscle protein degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of postmortem storage temperature on sea bass ( Dicentrarchus labrax ) muscle protein degradation : analysis by 2-D DIGE and MS .
	manualset3
237269	5	421842	7	NULL	NULL	0	NULL	 analysis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of postmortem storage temperature on sea bass ( Dicentrarchus labrax ) muscle protein degradation : analysis by 2-D DIGE and MS .
	manualset3
237270	6	421842	7	NULL	NULL	0	NULL	2-D DIGE	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of postmortem storage temperature on sea bass ( Dicentrarchus labrax ) muscle protein degradation : analysis by 2-D DIGE and MS .
	manualset3
237271	7	421842	7	NULL	NULL	0	NULL	MS	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Effects of postmortem storage temperature on sea bass ( Dicentrarchus labrax ) muscle protein degradation : analysis by 2-D DIGE and MS .
	manualset3
237272	1	421843	7	NULL	NULL	0	NULL	WHO classification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	WHO classification did not statistically significantly affect outcome .
	manualset3
237273	2	421843	7	NULL	NULL	0	NULL	outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	WHO classification did not statistically significantly affect outcome .
	manualset3
237274	1	421844	7	NULL	NULL	0	NULL	 progression	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The progression of neurologic symptomatology in the first 48 hours after cerebral infarction appears in more than one third of the patients causing greater morbidity and mortality .
	manualset3
237275	2	421844	7	NULL	NULL	0	NULL	neurologic symptomatology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The progression of neurologic symptomatology in the first 48 hours after cerebral infarction appears in more than one third of the patients causing greater morbidity and mortality .
	manualset3
237276	3	421844	7	NULL	NULL	0	NULL	 first 48 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The progression of neurologic symptomatology in the first 48 hours after cerebral infarction appears in more than one third of the patients causing greater morbidity and mortality .
	manualset3
237277	4	421844	7	NULL	NULL	0	NULL	cerebral infarction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The progression of neurologic symptomatology in the first 48 hours after cerebral infarction appears in more than one third of the patients causing greater morbidity and mortality .
	manualset3
237278	5	421844	7	NULL	NULL	0	NULL	one third 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The progression of neurologic symptomatology in the first 48 hours after cerebral infarction appears in more than one third of the patients causing greater morbidity and mortality .
	manualset3
237279	6	421844	7	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The progression of neurologic symptomatology in the first 48 hours after cerebral infarction appears in more than one third of the patients causing greater morbidity and mortality .
	manualset3
237280	7	421844	7	NULL	NULL	0	NULL	greater morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The progression of neurologic symptomatology in the first 48 hours after cerebral infarction appears in more than one third of the patients causing greater morbidity and mortality .
	manualset3
237281	8	421844	7	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The progression of neurologic symptomatology in the first 48 hours after cerebral infarction appears in more than one third of the patients causing greater morbidity and mortality .
	manualset3
237282	1	421845	7	NULL	NULL	NULL	NULL	gene	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Recently a gene which encodes a transmembrane serine protease , TMPRSS3 or ECHOS1 , was found to be responsible for both the DFNB8 and DFNB10 phenotypes .
	manualset3
237283	2	421845	7	NULL	NULL	0	NULL	 transmembrane serine protease	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently a gene which encodes a transmembrane serine protease , TMPRSS3 or ECHOS1 , was found to be responsible for both the DFNB8 and DFNB10 phenotypes .
	manualset3
237284	3	421845	7	NULL	NULL	0	NULL	TMPRSS3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently a gene which encodes a transmembrane serine protease , TMPRSS3 or ECHOS1 , was found to be responsible for both the DFNB8 and DFNB10 phenotypes .
	manualset3
237285	4	421845	7	NULL	NULL	0	NULL	ECHOS1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently a gene which encodes a transmembrane serine protease , TMPRSS3 or ECHOS1 , was found to be responsible for both the DFNB8 and DFNB10 phenotypes .
	manualset3
237286	5	421845	7	NULL	NULL	0	NULL	DFNB8 phenotypes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently a gene which encodes a transmembrane serine protease , TMPRSS3 or ECHOS1 , was found to be responsible for both the DFNB8 and DFNB10 phenotypes .
	manualset3
237287	6	421845	7	NULL	NULL	0	NULL	DFNB10 phenotypes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Recently a gene which encodes a transmembrane serine protease , TMPRSS3 or ECHOS1 , was found to be responsible for both the DFNB8 and DFNB10 phenotypes .
	manualset3
237289	1	421846	7	NULL	NULL	0	NULL	 technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique produced high yields of well-spread metaphases facilitating clonal cytogenetic analysis .
	manualset3
237290	2	421846	7	NULL	NULL	0	NULL	high yields	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique produced high yields of well-spread metaphases facilitating clonal cytogenetic analysis .
	manualset3
237291	3	421846	7	NULL	NULL	0	NULL	well-spread metaphases	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique produced high yields of well-spread metaphases facilitating clonal cytogenetic analysis .
	manualset3
237292	4	421846	7	NULL	NULL	0	NULL	clonal cytogenetic analysis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The technique produced high yields of well-spread metaphases facilitating clonal cytogenetic analysis .
	manualset3
237293	1	421847	7	NULL	NULL	0	NULL	cDNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The cDNA of a rat brain A1 adenosine receptor was stably expressed in CHO-cells , resulting in clones with varying receptor densities ; a clone expressing 1.9 pmol receptors/mg membrane protein was used for further characterization .
	manualset3
237294	2	421847	7	NULL	NULL	0	NULL	rat brain A1 adenosine receptor 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The cDNA of a rat brain A1 adenosine receptor was stably expressed in CHO-cells , resulting in clones with varying receptor densities ; a clone expressing 1.9 pmol receptors/mg membrane protein was used for further characterization .
	manualset3
237295	3	421847	7	NULL	NULL	0	NULL	CHO-cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The cDNA of a rat brain A1 adenosine receptor was stably expressed in CHO-cells , resulting in clones with varying receptor densities ; a clone expressing 1.9 pmol receptors/mg membrane protein was used for further characterization .
	manualset3
237296	4	421847	7	NULL	NULL	0	NULL	clones	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The cDNA of a rat brain A1 adenosine receptor was stably expressed in CHO-cells , resulting in clones with varying receptor densities ; a clone expressing 1.9 pmol receptors/mg membrane protein was used for further characterization .
	manualset3
237297	5	421847	7	NULL	NULL	0	NULL	receptor densities	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The cDNA of a rat brain A1 adenosine receptor was stably expressed in CHO-cells , resulting in clones with varying receptor densities ; a clone expressing 1.9 pmol receptors/mg membrane protein was used for further characterization .
	manualset3
237298	6	421847	7	NULL	NULL	0	NULL	clone	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The cDNA of a rat brain A1 adenosine receptor was stably expressed in CHO-cells , resulting in clones with varying receptor densities ; a clone expressing 1.9 pmol receptors/mg membrane protein was used for further characterization .
	manualset3
237299	7	421847	7	NULL	NULL	0	NULL	1.9 pmol receptors/mg membrane protein	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cDNA of a rat brain A1 adenosine receptor was stably expressed in CHO-cells , resulting in clones with varying receptor densities ; a clone expressing 1.9 pmol receptors/mg membrane protein was used for further characterization .
	manualset3
237300	8	421847	7	NULL	NULL	0	NULL	characterization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cDNA of a rat brain A1 adenosine receptor was stably expressed in CHO-cells , resulting in clones with varying receptor densities ; a clone expressing 1.9 pmol receptors/mg membrane protein was used for further characterization .
	manualset3
237301	1	421848	7	NULL	NULL	0	NULL	 ( - / - ) mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Them1 ( - / - ) mice exhibited increased O ( 2 ) consumption and heat production , which were accompanied by increased rates of fatty acid oxidation in brown adipose tissue and up-regulation of genes that promote energy expenditure .
	manualset3
237302	2	421848	7	NULL	NULL	0	NULL	O ( 2 ) consumption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Them1 ( - / - ) mice exhibited increased O ( 2 ) consumption and heat production , which were accompanied by increased rates of fatty acid oxidation in brown adipose tissue and up-regulation of genes that promote energy expenditure .
	manualset3
237303	3	421848	7	NULL	NULL	0	NULL	heat production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Them1 ( - / - ) mice exhibited increased O ( 2 ) consumption and heat production , which were accompanied by increased rates of fatty acid oxidation in brown adipose tissue and up-regulation of genes that promote energy expenditure .
	manualset3
237304	4	421848	7	NULL	NULL	0	NULL	 increased rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Them1 ( - / - ) mice exhibited increased O ( 2 ) consumption and heat production , which were accompanied by increased rates of fatty acid oxidation in brown adipose tissue and up-regulation of genes that promote energy expenditure .
	manualset3
237305	5	421848	7	NULL	NULL	0	NULL	fatty acid oxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Them1 ( - / - ) mice exhibited increased O ( 2 ) consumption and heat production , which were accompanied by increased rates of fatty acid oxidation in brown adipose tissue and up-regulation of genes that promote energy expenditure .
	manualset3
237306	6	421848	7	NULL	NULL	0	NULL	brown adipose tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Them1 ( - / - ) mice exhibited increased O ( 2 ) consumption and heat production , which were accompanied by increased rates of fatty acid oxidation in brown adipose tissue and up-regulation of genes that promote energy expenditure .
	manualset3
237307	7	421848	7	NULL	NULL	0	NULL	up-regulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Them1 ( - / - ) mice exhibited increased O ( 2 ) consumption and heat production , which were accompanied by increased rates of fatty acid oxidation in brown adipose tissue and up-regulation of genes that promote energy expenditure .
	manualset3
237308	8	421848	7	NULL	NULL	0	NULL	genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Them1 ( - / - ) mice exhibited increased O ( 2 ) consumption and heat production , which were accompanied by increased rates of fatty acid oxidation in brown adipose tissue and up-regulation of genes that promote energy expenditure .
	manualset3
237309	9	421848	7	NULL	NULL	0	NULL	energy expenditure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Them1 ( - / - ) mice exhibited increased O ( 2 ) consumption and heat production , which were accompanied by increased rates of fatty acid oxidation in brown adipose tissue and up-regulation of genes that promote energy expenditure .
	manualset3
237316	1	421849	7	NULL	NULL	0	NULL	Radiologic aspects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiologic aspects of arteriovenous aneurysm of the great vein of Galen .
	manualset3
237317	2	421849	7	NULL	NULL	0	NULL	arteriovenous aneurysm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Radiologic aspects of arteriovenous aneurysm of the great vein of Galen .
	manualset3
237318	3	421849	7	NULL	NULL	NULL	NULL	great vein of Galen	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Radiologic aspects of arteriovenous aneurysm of the great vein of Galen .
	manualset3
237319	1	421850	7	NULL	NULL	0	NULL	gonadotropin-induced increase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The gonadotropin-induced increase in HMG CoA reductase activity seemed to be due to a net increase in enzyme activity , not to a change in the phosphorylated/dephosphorylated state of the enzyme .
	manualset3
237320	2	421850	7	NULL	NULL	0	NULL	HMG CoA reductase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The gonadotropin-induced increase in HMG CoA reductase activity seemed to be due to a net increase in enzyme activity , not to a change in the phosphorylated/dephosphorylated state of the enzyme .
	manualset3
237321	3	421850	7	NULL	NULL	0	NULL	net increase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The gonadotropin-induced increase in HMG CoA reductase activity seemed to be due to a net increase in enzyme activity , not to a change in the phosphorylated/dephosphorylated state of the enzyme .
	manualset3
237322	4	421850	7	NULL	NULL	0	NULL	 enzyme activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The gonadotropin-induced increase in HMG CoA reductase activity seemed to be due to a net increase in enzyme activity , not to a change in the phosphorylated/dephosphorylated state of the enzyme .
	manualset3
237323	5	421850	7	NULL	NULL	0	NULL	change	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The gonadotropin-induced increase in HMG CoA reductase activity seemed to be due to a net increase in enzyme activity , not to a change in the phosphorylated/dephosphorylated state of the enzyme .
	manualset3
237324	6	421850	7	NULL	NULL	0	NULL	phosphorylated/dephosphorylated state	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The gonadotropin-induced increase in HMG CoA reductase activity seemed to be due to a net increase in enzyme activity , not to a change in the phosphorylated/dephosphorylated state of the enzyme .
	manualset3
237325	7	421850	7	NULL	NULL	0	NULL	enzyme 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The gonadotropin-induced increase in HMG CoA reductase activity seemed to be due to a net increase in enzyme activity , not to a change in the phosphorylated/dephosphorylated state of the enzyme .
	manualset3
237380	1	421851	7	NULL	NULL	0	NULL	 early decrease	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An early decrease in interphotoreceptor retinoid-binding protein gene expression in Abyssinian cats homozygous for hereditary rod-cone degeneration .
	manualset3
237382	2	421851	7	NULL	NULL	0	NULL	interphotoreceptor retinoid-binding protein gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An early decrease in interphotoreceptor retinoid-binding protein gene expression in Abyssinian cats homozygous for hereditary rod-cone degeneration .
	manualset3
237383	3	421851	7	NULL	NULL	0	NULL	Abyssinian cats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	An early decrease in interphotoreceptor retinoid-binding protein gene expression in Abyssinian cats homozygous for hereditary rod-cone degeneration .
	manualset3
237384	4	421851	7	NULL	NULL	0	NULL	hereditary rod-cone degeneration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An early decrease in interphotoreceptor retinoid-binding protein gene expression in Abyssinian cats homozygous for hereditary rod-cone degeneration .
	manualset3
237393	1	421852	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to patients with sudden coronary death and acute myocardial infarction , relatively little morphologic data has been reported in patients with unstable angina pectoris .
	manualset3
237399	2	421852	7	NULL	NULL	0	NULL	sudden coronary death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to patients with sudden coronary death and acute myocardial infarction , relatively little morphologic data has been reported in patients with unstable angina pectoris .
	manualset3
237401	3	421852	7	NULL	NULL	0	NULL	acute myocardial infarction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to patients with sudden coronary death and acute myocardial infarction , relatively little morphologic data has been reported in patients with unstable angina pectoris .
	manualset3
237403	4	421852	7	NULL	NULL	0	NULL	morphologic data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to patients with sudden coronary death and acute myocardial infarction , relatively little morphologic data has been reported in patients with unstable angina pectoris .
	manualset3
237405	5	421852	7	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to patients with sudden coronary death and acute myocardial infarction , relatively little morphologic data has been reported in patients with unstable angina pectoris .
	manualset3
237406	6	421852	7	NULL	NULL	0	NULL	unstable angina pectoris	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to patients with sudden coronary death and acute myocardial infarction , relatively little morphologic data has been reported in patients with unstable angina pectoris .
	manualset3
237428	1	421853	7	NULL	NULL	0	NULL	Histamine H1 receptor antagonists 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Histamine H1 receptor antagonists inhibiting the LPR have a property distinct from H1 receptor antagonism , which may have an additional benefit for the treatment of allergic diseases .
	manualset3
237430	2	421853	7	NULL	NULL	0	NULL	LPR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Histamine H1 receptor antagonists inhibiting the LPR have a property distinct from H1 receptor antagonism , which may have an additional benefit for the treatment of allergic diseases .
	manualset3
237432	3	421853	7	NULL	NULL	0	NULL	H1 receptor antagonism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Histamine H1 receptor antagonists inhibiting the LPR have a property distinct from H1 receptor antagonism , which may have an additional benefit for the treatment of allergic diseases .
	manualset3
237433	4	421853	7	NULL	NULL	0	NULL	 treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Histamine H1 receptor antagonists inhibiting the LPR have a property distinct from H1 receptor antagonism , which may have an additional benefit for the treatment of allergic diseases .
	manualset3
237434	5	421853	7	NULL	NULL	0	NULL	allergic diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Histamine H1 receptor antagonists inhibiting the LPR have a property distinct from H1 receptor antagonism , which may have an additional benefit for the treatment of allergic diseases .
	manualset3
237445	1	421854	7	NULL	NULL	0	NULL	microvascularization abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The microvascularization abnormalities observed were mild and non specific .
	manualset3
237450	1	421855	7	NULL	NULL	0	NULL	behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The behavior of plasma tocopherol after the parenteral administration of tocopherol acetate in healthy subjects and in subjects with hyperthyroidism ) .
	manualset3
237452	2	421855	7	NULL	NULL	NULL	NULL	plasma tocopherol	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The behavior of plasma tocopherol after the parenteral administration of tocopherol acetate in healthy subjects and in subjects with hyperthyroidism ) .
	manualset3
237453	3	421855	7	NULL	NULL	0	NULL	parenteral administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( The behavior of plasma tocopherol after the parenteral administration of tocopherol acetate in healthy subjects and in subjects with hyperthyroidism ) .
	manualset3
237454	4	421855	7	NULL	NULL	NULL	NULL	 tocopherol acetate	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The behavior of plasma tocopherol after the parenteral administration of tocopherol acetate in healthy subjects and in subjects with hyperthyroidism ) .
	manualset3
237455	5	421855	7	NULL	NULL	0	NULL	healthy subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( The behavior of plasma tocopherol after the parenteral administration of tocopherol acetate in healthy subjects and in subjects with hyperthyroidism ) .
	manualset3
237457	6	421855	7	NULL	NULL	0	NULL	 subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( The behavior of plasma tocopherol after the parenteral administration of tocopherol acetate in healthy subjects and in subjects with hyperthyroidism ) .
	manualset3
237458	7	421855	7	NULL	NULL	0	NULL	hyperthyroidism	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( The behavior of plasma tocopherol after the parenteral administration of tocopherol acetate in healthy subjects and in subjects with hyperthyroidism ) .
	manualset3
237461	1	421856	7	NULL	NULL	0	NULL	BLM	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	BLM , the structural gene mutated in individuals with the disorder , encodes a DNA helicase belonging to the RecQ family of helicases .
	manualset3
237462	2	421856	7	NULL	NULL	0	NULL	structural gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	BLM , the structural gene mutated in individuals with the disorder , encodes a DNA helicase belonging to the RecQ family of helicases .
	manualset3
237463	3	421856	7	NULL	NULL	0	NULL	 individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	BLM , the structural gene mutated in individuals with the disorder , encodes a DNA helicase belonging to the RecQ family of helicases .
	manualset3
237466	4	421856	7	NULL	NULL	0	NULL	disorder	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	BLM , the structural gene mutated in individuals with the disorder , encodes a DNA helicase belonging to the RecQ family of helicases .
	manualset3
237468	5	421856	7	NULL	NULL	0	NULL	DNA helicase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	BLM , the structural gene mutated in individuals with the disorder , encodes a DNA helicase belonging to the RecQ family of helicases .
	manualset3
237470	6	421856	7	NULL	NULL	0	NULL	RecQ family 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	BLM , the structural gene mutated in individuals with the disorder , encodes a DNA helicase belonging to the RecQ family of helicases .
	manualset3
237473	7	421856	7	NULL	NULL	0	NULL	helicases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	BLM , the structural gene mutated in individuals with the disorder , encodes a DNA helicase belonging to the RecQ family of helicases .
	manualset3
237475	1	421857	7	NULL	NULL	0	NULL	SPARC binding sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Identifying the SPARC binding sites on collagen I and procollagen I by atomic force microscopy .
	manualset3
237478	2	421857	7	NULL	NULL	0	NULL	collagen I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Identifying the SPARC binding sites on collagen I and procollagen I by atomic force microscopy .
	manualset3
237480	3	421857	7	NULL	NULL	0	NULL	procollagen I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Identifying the SPARC binding sites on collagen I and procollagen I by atomic force microscopy .
	manualset3
237481	4	421857	7	NULL	NULL	0	NULL	atomic force microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Identifying the SPARC binding sites on collagen I and procollagen I by atomic force microscopy .
	manualset3
237484	1	421858	7	NULL	NULL	NULL	NULL	early signal	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An early signal of synaptosomal apoptosis is the loss of phospholipid asymmetry and the appearance of phosphatidylserine ( PS ) in the outer leaflet of the membrane .
	manualset3
237485	2	421858	7	NULL	NULL	0	NULL	synaptosomal apoptosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An early signal of synaptosomal apoptosis is the loss of phospholipid asymmetry and the appearance of phosphatidylserine ( PS ) in the outer leaflet of the membrane .
	manualset3
237486	3	421858	7	NULL	NULL	0	NULL	 loss	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An early signal of synaptosomal apoptosis is the loss of phospholipid asymmetry and the appearance of phosphatidylserine ( PS ) in the outer leaflet of the membrane .
	manualset3
237487	4	421858	7	NULL	NULL	0	NULL	phospholipid asymmetry	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An early signal of synaptosomal apoptosis is the loss of phospholipid asymmetry and the appearance of phosphatidylserine ( PS ) in the outer leaflet of the membrane .
	manualset3
237488	5	421858	7	NULL	NULL	0	NULL	phosphatidylserine ( PS )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An early signal of synaptosomal apoptosis is the loss of phospholipid asymmetry and the appearance of phosphatidylserine ( PS ) in the outer leaflet of the membrane .
	manualset3
237489	6	421858	7	NULL	NULL	0	NULL	 outer leaflet	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	An early signal of synaptosomal apoptosis is the loss of phospholipid asymmetry and the appearance of phosphatidylserine ( PS ) in the outer leaflet of the membrane .
	manualset3
237490	7	421858	7	NULL	NULL	0	NULL	membrane 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	An early signal of synaptosomal apoptosis is the loss of phospholipid asymmetry and the appearance of phosphatidylserine ( PS ) in the outer leaflet of the membrane .
	manualset3
237491	1	421859	7	NULL	NULL	0	NULL	Clinical experience	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical experience with a combination of bupivacaine and buprenorphine for subarachnoid anesthesia in orthopedic-traumatologic surgery in the elderly patient ) .
	manualset3
237492	2	421859	7	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical experience with a combination of bupivacaine and buprenorphine for subarachnoid anesthesia in orthopedic-traumatologic surgery in the elderly patient ) .
	manualset3
237493	3	421859	7	NULL	NULL	NULL	NULL	bupivacaine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Clinical experience with a combination of bupivacaine and buprenorphine for subarachnoid anesthesia in orthopedic-traumatologic surgery in the elderly patient ) .
	manualset3
237494	4	421859	7	NULL	NULL	NULL	NULL	buprenorphine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Clinical experience with a combination of bupivacaine and buprenorphine for subarachnoid anesthesia in orthopedic-traumatologic surgery in the elderly patient ) .
	manualset3
237495	5	421859	7	NULL	NULL	0	NULL	subarachnoid anesthesia	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical experience with a combination of bupivacaine and buprenorphine for subarachnoid anesthesia in orthopedic-traumatologic surgery in the elderly patient ) .
	manualset3
237496	6	421859	7	NULL	NULL	0	NULL	orthopedic-traumatologic surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical experience with a combination of bupivacaine and buprenorphine for subarachnoid anesthesia in orthopedic-traumatologic surgery in the elderly patient ) .
	manualset3
237497	7	421859	7	NULL	NULL	0	NULL	elderly patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinical experience with a combination of bupivacaine and buprenorphine for subarachnoid anesthesia in orthopedic-traumatologic surgery in the elderly patient ) .
	manualset3
237498	1	421860	7	NULL	NULL	0	NULL	Cytokinesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cytokinesis is the last step of cell division that physically separates the daughter cells .
	manualset3
237499	2	421860	7	NULL	NULL	0	NULL	 last step	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cytokinesis is the last step of cell division that physically separates the daughter cells .
	manualset3
237500	3	421860	7	NULL	NULL	0	NULL	cell division 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cytokinesis is the last step of cell division that physically separates the daughter cells .
	manualset3
237501	4	421860	7	NULL	NULL	0	NULL	daughter cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Cytokinesis is the last step of cell division that physically separates the daughter cells .
	manualset3
237502	1	421861	7	NULL	NULL	0	NULL	reciprocal fusion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The reciprocal fusion , which would contain the p53-binding 53BP1 BRCA1 COOH-terminal domains , was not detectable by fluorescence in situ hybridization or nested PCR .
	manualset3
237503	2	421861	7	NULL	NULL	0	NULL	p53-binding 53BP1 BRCA1 COOH-terminal domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The reciprocal fusion , which would contain the p53-binding 53BP1 BRCA1 COOH-terminal domains , was not detectable by fluorescence in situ hybridization or nested PCR .
	manualset3
237504	3	421861	7	NULL	NULL	NULL	NULL	 fluorescence  in situ hybridization 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reciprocal fusion , which would contain the p53-binding 53BP1 BRCA1 COOH-terminal domains , was not detectable by fluorescence in situ hybridization or nested PCR .
	manualset3
237505	4	421861	7	NULL	NULL	0	NULL	nested PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The reciprocal fusion , which would contain the p53-binding 53BP1 BRCA1 COOH-terminal domains , was not detectable by fluorescence in situ hybridization or nested PCR .
	manualset3
237506	1	421862	7	NULL	NULL	0	NULL	method	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is demonstrated with isokinetic shear flow , in bulk and slit geometries , which illustrates its flexibility .
	manualset3
237507	2	421862	7	NULL	NULL	0	NULL	isokinetic shear flow	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is demonstrated with isokinetic shear flow , in bulk and slit geometries , which illustrates its flexibility .
	manualset3
237508	3	421862	7	NULL	NULL	0	NULL	 slit geometries	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is demonstrated with isokinetic shear flow , in bulk and slit geometries , which illustrates its flexibility .
	manualset3
237509	4	421862	7	NULL	NULL	0	NULL	 flexibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The method is demonstrated with isokinetic shear flow , in bulk and slit geometries , which illustrates its flexibility .
	manualset3
237581	1	421863	7	NULL	NULL	0	NULL	Oral antibiotic treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral antibiotic treatment of Helicobacter pylori leads to persistently reduced intestinal colonization rates with oxalobacter formigenes .
	manualset3
237583	2	421863	7	NULL	NULL	0	NULL	Helicobacter pylori 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral antibiotic treatment of Helicobacter pylori leads to persistently reduced intestinal colonization rates with oxalobacter formigenes .
	manualset3
237585	3	421863	7	NULL	NULL	0	NULL	intestinal colonization rates	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral antibiotic treatment of Helicobacter pylori leads to persistently reduced intestinal colonization rates with oxalobacter formigenes .
	manualset3
237719	4	421863	7	NULL	NULL	0	NULL	oxalobacter formigenes 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Oral antibiotic treatment of Helicobacter pylori leads to persistently reduced intestinal colonization rates with oxalobacter formigenes .
	manualset3
237723	1	421864	7	NULL	NULL	0	NULL	plasmafiltration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from plasmafiltration , treatment with azathioprim and steroids proved to be effective .
	manualset3
237725	2	421864	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from plasmafiltration , treatment with azathioprim and steroids proved to be effective .
	manualset3
237727	3	421864	7	NULL	NULL	0	NULL	azathioprim	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from plasmafiltration , treatment with azathioprim and steroids proved to be effective .
	manualset3
237728	4	421864	7	NULL	NULL	0	NULL	steroids	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from plasmafiltration , treatment with azathioprim and steroids proved to be effective .
	manualset3
237732	1	421865	7	NULL	NULL	0	NULL	 source reconstruction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The accuracy of source reconstruction appears to be more related to depth than source orientation .
	manualset3
237733	2	421865	7	NULL	NULL	0	NULL	depth 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The accuracy of source reconstruction appears to be more related to depth than source orientation .
	manualset3
237734	3	421865	7	NULL	NULL	0	NULL	source orientation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The accuracy of source reconstruction appears to be more related to depth than source orientation .
	manualset3
243953	4	421865	7	NULL	NULL	0	NULL	 accuracy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The accuracy of source reconstruction appears to be more related to depth than source orientation .
	manualset3
237742	1	421866	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Among all patients , left ventricular dilatation carried a relative risk of myocardial infarction of 5.8 ; low ejection fraction and right ventricular dilatation were strongly associated with myocardial infarction .
	manualset3
237744	2	421866	7	NULL	NULL	0	NULL	left ventricular dilatation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Among all patients , left ventricular dilatation carried a relative risk of myocardial infarction of 5.8 ; low ejection fraction and right ventricular dilatation were strongly associated with myocardial infarction .
	manualset3
237745	3	421866	7	NULL	NULL	0	NULL	relative risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among all patients , left ventricular dilatation carried a relative risk of myocardial infarction of 5.8 ; low ejection fraction and right ventricular dilatation were strongly associated with myocardial infarction .
	manualset3
237747	4	421866	7	NULL	NULL	0	NULL	myocardial infarction	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Among all patients , left ventricular dilatation carried a relative risk of myocardial infarction of 5.8 ; low ejection fraction and right ventricular dilatation were strongly associated with myocardial infarction .
	manualset3
237749	5	421866	7	NULL	NULL	0	NULL	5.8 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Among all patients , left ventricular dilatation carried a relative risk of myocardial infarction of 5.8 ; low ejection fraction and right ventricular dilatation were strongly associated with myocardial infarction .
	manualset3
237750	6	421866	7	NULL	NULL	0	NULL	low ejection fraction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among all patients , left ventricular dilatation carried a relative risk of myocardial infarction of 5.8 ; low ejection fraction and right ventricular dilatation were strongly associated with myocardial infarction .
	manualset3
237752	7	421866	7	NULL	NULL	NULL	NULL	right ventricular dilatation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Among all patients , left ventricular dilatation carried a relative risk of myocardial infarction of 5.8 ; low ejection fraction and right ventricular dilatation were strongly associated with myocardial infarction .
	manualset3
237753	8	421866	7	NULL	NULL	0	NULL	myocardial infarction	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Among all patients , left ventricular dilatation carried a relative risk of myocardial infarction of 5.8 ; low ejection fraction and right ventricular dilatation were strongly associated with myocardial infarction .
	manualset3
237761	1	421867	7	NULL	NULL	0	NULL	inexpensive procedure 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An easy and inexpensive procedure is described for the quantitative removal of SpA from TCGF without loss of TCGF activity .
	manualset3
237762	2	421867	7	NULL	NULL	0	NULL	 quantitative removal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An easy and inexpensive procedure is described for the quantitative removal of SpA from TCGF without loss of TCGF activity .
	manualset3
237763	3	421867	7	NULL	NULL	0	NULL	SpA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	An easy and inexpensive procedure is described for the quantitative removal of SpA from TCGF without loss of TCGF activity .
	manualset3
237764	4	421867	7	NULL	NULL	0	NULL	TCGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	An easy and inexpensive procedure is described for the quantitative removal of SpA from TCGF without loss of TCGF activity .
	manualset3
237765	5	421867	7	NULL	NULL	0	NULL	loss	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An easy and inexpensive procedure is described for the quantitative removal of SpA from TCGF without loss of TCGF activity .
	manualset3
237766	6	421867	7	NULL	NULL	0	NULL	TCGF activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An easy and inexpensive procedure is described for the quantitative removal of SpA from TCGF without loss of TCGF activity .
	manualset3
237767	1	421868	7	NULL	NULL	0	NULL	frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of the new platelet antigen Cab in the Brazilian population .
	manualset3
237769	2	421868	7	NULL	NULL	0	NULL	new platelet antigen Cab	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of the new platelet antigen Cab in the Brazilian population .
	manualset3
237770	3	421868	7	NULL	NULL	0	NULL	Brazilian population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of the new platelet antigen Cab in the Brazilian population .
	manualset3
237888	1	421869	7	NULL	NULL	0	NULL	usage 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the usage of arginine residues in voltage sensors is an adaptation to the phospholipid composition of cell membranes .
	manualset3
237889	2	421869	7	NULL	NULL	0	NULL	arginine residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the usage of arginine residues in voltage sensors is an adaptation to the phospholipid composition of cell membranes .
	manualset3
237890	3	421869	7	NULL	NULL	0	NULL	voltage sensors	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the usage of arginine residues in voltage sensors is an adaptation to the phospholipid composition of cell membranes .
	manualset3
237891	4	421869	7	NULL	NULL	0	NULL	adaptation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the usage of arginine residues in voltage sensors is an adaptation to the phospholipid composition of cell membranes .
	manualset3
237892	5	421869	7	NULL	NULL	0	NULL	phospholipid composition	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the usage of arginine residues in voltage sensors is an adaptation to the phospholipid composition of cell membranes .
	manualset3
237893	6	421869	7	NULL	NULL	0	NULL	cell membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	We suggest that the usage of arginine residues in voltage sensors is an adaptation to the phospholipid composition of cell membranes .
	manualset3
237894	1	421870	7	NULL	NULL	0	NULL	Effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of electric fields on performance and affect in healthy probands ) .
	manualset3
237895	2	421870	7	NULL	NULL	0	NULL	electric fields	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of electric fields on performance and affect in healthy probands ) .
	manualset3
237896	3	421870	7	NULL	NULL	0	NULL	healthy probands	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of electric fields on performance and affect in healthy probands ) .
	manualset3
237897	1	421871	7	NULL	NULL	0	NULL	three OP compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All three OP compounds inhibited the CaM activity and its active conformation in a concentration-dependent manner .
	manualset3
237898	2	421871	7	NULL	NULL	0	NULL	CaM activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All three OP compounds inhibited the CaM activity and its active conformation in a concentration-dependent manner .
	manualset3
237899	3	421871	7	NULL	NULL	0	NULL	active conformation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All three OP compounds inhibited the CaM activity and its active conformation in a concentration-dependent manner .
	manualset3
237900	4	421871	7	NULL	NULL	0	NULL	concentration-dependent manner	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	All three OP compounds inhibited the CaM activity and its active conformation in a concentration-dependent manner .
	manualset3
237901	1	421872	7	NULL	NULL	0	NULL	gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene coding for the N protein of RSV strain Long has been cloned and sequenced .
	manualset3
237902	2	421872	7	NULL	NULL	0	NULL	 N protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene coding for the N protein of RSV strain Long has been cloned and sequenced .
	manualset3
237903	3	421872	7	NULL	NULL	0	NULL	RSV strain Long	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The gene coding for the N protein of RSV strain Long has been cloned and sequenced .
	manualset3
237904	1	421873	7	NULL	NULL	0	NULL	partial thromboplastin time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Decrease in partial thromboplastin time , increase in plasma fibrinogen and platelet count , and reduction in clot retraction indicate a hypercoagulable state .
	manualset3
237905	2	421873	7	NULL	NULL	0	NULL	plasma fibrinogen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Decrease in partial thromboplastin time , increase in plasma fibrinogen and platelet count , and reduction in clot retraction indicate a hypercoagulable state .
	manualset3
237906	3	421873	7	NULL	NULL	0	NULL	platelet count	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Decrease in partial thromboplastin time , increase in plasma fibrinogen and platelet count , and reduction in clot retraction indicate a hypercoagulable state .
	manualset3
237907	4	421873	7	NULL	NULL	0	NULL	reduction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Decrease in partial thromboplastin time , increase in plasma fibrinogen and platelet count , and reduction in clot retraction indicate a hypercoagulable state .
	manualset3
237908	5	421873	7	NULL	NULL	0	NULL	clot retraction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Decrease in partial thromboplastin time , increase in plasma fibrinogen and platelet count , and reduction in clot retraction indicate a hypercoagulable state .
	manualset3
237909	6	421873	7	NULL	NULL	0	NULL	hypercoagulable state .	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Decrease in partial thromboplastin time , increase in plasma fibrinogen and platelet count , and reduction in clot retraction indicate a hypercoagulable state .
	manualset3
237910	1	421874	7	NULL	NULL	0	NULL	PGS	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is demonstrated that PGS is sufficiently permeable to water to allow the design of an elementary osmotic pump for drug delivery .
	manualset3
237911	2	421874	7	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	It is demonstrated that PGS is sufficiently permeable to water to allow the design of an elementary osmotic pump for drug delivery .
	manualset3
237912	3	421874	7	NULL	NULL	0	NULL	design	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is demonstrated that PGS is sufficiently permeable to water to allow the design of an elementary osmotic pump for drug delivery .
	manualset3
237913	4	421874	7	NULL	NULL	0	NULL	elementary osmotic pump 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	It is demonstrated that PGS is sufficiently permeable to water to allow the design of an elementary osmotic pump for drug delivery .
	manualset3
237914	5	421874	7	NULL	NULL	0	NULL	drug delivery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	It is demonstrated that PGS is sufficiently permeable to water to allow the design of an elementary osmotic pump for drug delivery .
	manualset3
237915	1	421875	7	NULL	NULL	0	NULL	 findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings need to be interpreted with caution given the heterogeneity between studies , as well as the attenuation of the risk estimates in analyses that attempted to control for the unmeasured characteristics of areas with high levels of income inequality .
	manualset3
237916	2	421875	7	NULL	NULL	0	NULL	caution	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings need to be interpreted with caution given the heterogeneity between studies , as well as the attenuation of the risk estimates in analyses that attempted to control for the unmeasured characteristics of areas with high levels of income inequality .
	manualset3
237917	3	421875	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings need to be interpreted with caution given the heterogeneity between studies , as well as the attenuation of the risk estimates in analyses that attempted to control for the unmeasured characteristics of areas with high levels of income inequality .
	manualset3
237918	4	421875	7	NULL	NULL	0	NULL	attenuation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings need to be interpreted with caution given the heterogeneity between studies , as well as the attenuation of the risk estimates in analyses that attempted to control for the unmeasured characteristics of areas with high levels of income inequality .
	manualset3
237919	5	421875	7	NULL	NULL	NULL	NULL	risk estimates	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The findings need to be interpreted with caution given the heterogeneity between studies , as well as the attenuation of the risk estimates in analyses that attempted to control for the unmeasured characteristics of areas with high levels of income inequality .
	manualset3
237920	6	421875	7	NULL	NULL	0	NULL	analyses 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings need to be interpreted with caution given the heterogeneity between studies , as well as the attenuation of the risk estimates in analyses that attempted to control for the unmeasured characteristics of areas with high levels of income inequality .
	manualset3
237921	7	421875	7	NULL	NULL	0	NULL	areas	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings need to be interpreted with caution given the heterogeneity between studies , as well as the attenuation of the risk estimates in analyses that attempted to control for the unmeasured characteristics of areas with high levels of income inequality .
	manualset3
237922	8	421875	7	NULL	NULL	0	NULL	high levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings need to be interpreted with caution given the heterogeneity between studies , as well as the attenuation of the risk estimates in analyses that attempted to control for the unmeasured characteristics of areas with high levels of income inequality .
	manualset3
237923	9	421875	7	NULL	NULL	0	NULL	income inequality	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings need to be interpreted with caution given the heterogeneity between studies , as well as the attenuation of the risk estimates in analyses that attempted to control for the unmeasured characteristics of areas with high levels of income inequality .
	manualset3
237924	10	421875	7	NULL	NULL	0	NULL	unmeasured characteristics	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings need to be interpreted with caution given the heterogeneity between studies , as well as the attenuation of the risk estimates in analyses that attempted to control for the unmeasured characteristics of areas with high levels of income inequality .
	manualset3
242840	11	421875	7	NULL	NULL	0	NULL	heterogeneity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings need to be interpreted with caution given the heterogeneity between studies , as well as the attenuation of the risk estimates in analyses that attempted to control for the unmeasured characteristics of areas with high levels of income inequality .
	manualset3
237925	1	421876	7	NULL	NULL	0	NULL	Clinical studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical studies indicate that intramyocardial injection of autologous cells to augment contractile function may modify the arrhythmogenic substrate .
	manualset3
237926	2	421876	7	NULL	NULL	0	NULL	intramyocardial injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical studies indicate that intramyocardial injection of autologous cells to augment contractile function may modify the arrhythmogenic substrate .
	manualset3
237927	3	421876	7	NULL	NULL	0	NULL	autologous cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical studies indicate that intramyocardial injection of autologous cells to augment contractile function may modify the arrhythmogenic substrate .
	manualset3
237928	4	421876	7	NULL	NULL	0	NULL	contractile function 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical studies indicate that intramyocardial injection of autologous cells to augment contractile function may modify the arrhythmogenic substrate .
	manualset3
237929	5	421876	7	NULL	NULL	0	NULL	arrhythmogenic substrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Clinical studies indicate that intramyocardial injection of autologous cells to augment contractile function may modify the arrhythmogenic substrate .
	manualset3
237930	1	421877	7	NULL	NULL	0	NULL	( 4 +1 ) cycloaddition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An efficient , overall ( 4 +1 ) cycloaddition of 1 , 3-dienes and nitrene precursors .
	manualset3
237931	2	421877	7	NULL	NULL	0	NULL	 1 , 3-dienes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An efficient , overall ( 4 +1 ) cycloaddition of 1 , 3-dienes and nitrene precursors .
	manualset3
237932	3	421877	7	NULL	NULL	0	NULL	nitrene precursors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An efficient , overall ( 4 +1 ) cycloaddition of 1 , 3-dienes and nitrene precursors .
	manualset3
237933	1	421878	7	NULL	NULL	0	NULL	2x taxa 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2x taxa while showing close relation among themselves are sharply segregated from 4x and 6x taxa belonging to C. album and C. giganteum .
	manualset3
237934	2	421878	7	NULL	NULL	0	NULL	close relation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2x taxa while showing close relation among themselves are sharply segregated from 4x and 6x taxa belonging to C. album and C. giganteum .
	manualset3
237935	3	421878	7	NULL	NULL	0	NULL	4x taxa	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2x taxa while showing close relation among themselves are sharply segregated from 4x and 6x taxa belonging to C. album and C. giganteum .
	manualset3
237936	4	421878	7	NULL	NULL	0	NULL	6x taxa	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2x taxa while showing close relation among themselves are sharply segregated from 4x and 6x taxa belonging to C. album and C. giganteum .
	manualset3
237937	5	421878	7	NULL	NULL	0	NULL	C. album	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2x taxa while showing close relation among themselves are sharply segregated from 4x and 6x taxa belonging to C. album and C. giganteum .
	manualset3
242853	6	421878	7	NULL	NULL	0	NULL	C. giganteum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The 2x taxa while showing close relation among themselves are sharply segregated from 4x and 6x taxa belonging to C. album and C. giganteum .
	manualset3
237938	1	421879	7	NULL	NULL	0	NULL	conclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the methods developed allowed for reproducible quantification of Cl ( biliary ) of drugs in healthy humans and prediction of Cl ( biliary ) from in vitro data .
	manualset3
237939	2	421879	7	NULL	NULL	0	NULL	methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the methods developed allowed for reproducible quantification of Cl ( biliary ) of drugs in healthy humans and prediction of Cl ( biliary ) from in vitro data .
	manualset3
237940	3	421879	7	NULL	NULL	0	NULL	reproducible quantification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the methods developed allowed for reproducible quantification of Cl ( biliary ) of drugs in healthy humans and prediction of Cl ( biliary ) from in vitro data .
	manualset3
237941	4	421879	7	NULL	NULL	0	NULL	Cl ( biliary )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the methods developed allowed for reproducible quantification of Cl ( biliary ) of drugs in healthy humans and prediction of Cl ( biliary ) from in vitro data .
	manualset3
237942	5	421879	7	NULL	NULL	0	NULL	drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the methods developed allowed for reproducible quantification of Cl ( biliary ) of drugs in healthy humans and prediction of Cl ( biliary ) from in vitro data .
	manualset3
237943	6	421879	7	NULL	NULL	0	NULL	healthy humans 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the methods developed allowed for reproducible quantification of Cl ( biliary ) of drugs in healthy humans and prediction of Cl ( biliary ) from in vitro data .
	manualset3
237944	7	421879	7	NULL	NULL	0	NULL	 prediction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the methods developed allowed for reproducible quantification of Cl ( biliary ) of drugs in healthy humans and prediction of Cl ( biliary ) from in vitro data .
	manualset3
237945	8	421879	7	NULL	NULL	0	NULL	Cl ( biliary )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the methods developed allowed for reproducible quantification of Cl ( biliary ) of drugs in healthy humans and prediction of Cl ( biliary ) from in vitro data .
	manualset3
237946	9	421879	7	NULL	NULL	0	NULL	in vitro data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In conclusion , the methods developed allowed for reproducible quantification of Cl ( biliary ) of drugs in healthy humans and prediction of Cl ( biliary ) from in vitro data .
	manualset3
237947	1	421880	7	NULL	NULL	0	NULL	Amniotic fluid index 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Amniotic fluid index during labor in women with EPH gestosis ) .
	manualset3
237948	2	421880	7	NULL	NULL	0	NULL	labor	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Amniotic fluid index during labor in women with EPH gestosis ) .
	manualset3
237949	3	421880	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Amniotic fluid index during labor in women with EPH gestosis ) .
	manualset3
237950	4	421880	7	NULL	NULL	0	NULL	EPH gestosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Amniotic fluid index during labor in women with EPH gestosis ) .
	manualset3
237951	1	421881	7	NULL	NULL	0	NULL	 discharge	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	At discharge , 638 ( 61 % ) patients received prescription for extended pharmacological prophylaxis : 564 ( 77 % ) after orthopaedic surgery , and 74 ( 23 % ) after cancer surgery ( p & lt ; 0.001 ) .
	manualset3
237952	2	421881	7	NULL	NULL	0	NULL	638 ( 61 % ) patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	At discharge , 638 ( 61 % ) patients received prescription for extended pharmacological prophylaxis : 564 ( 77 % ) after orthopaedic surgery , and 74 ( 23 % ) after cancer surgery ( p & lt ; 0.001 ) .
	manualset3
237954	3	421881	7	NULL	NULL	0	NULL	prescription	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	At discharge , 638 ( 61 % ) patients received prescription for extended pharmacological prophylaxis : 564 ( 77 % ) after orthopaedic surgery , and 74 ( 23 % ) after cancer surgery ( p & lt ; 0.001 ) .
	manualset3
237955	4	421881	7	NULL	NULL	0	NULL	extended pharmacological prophylaxis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	At discharge , 638 ( 61 % ) patients received prescription for extended pharmacological prophylaxis : 564 ( 77 % ) after orthopaedic surgery , and 74 ( 23 % ) after cancer surgery ( p & lt ; 0.001 ) .
	manualset3
237989	5	421881	7	NULL	NULL	0	NULL	 564	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	At discharge , 638 ( 61 % ) patients received prescription for extended pharmacological prophylaxis : 564 ( 77 % ) after orthopaedic surgery , and 74 ( 23 % ) after cancer surgery ( p & lt ; 0.001 ) .
	manualset3
237990	6	421881	7	NULL	NULL	0	NULL	77 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	At discharge , 638 ( 61 % ) patients received prescription for extended pharmacological prophylaxis : 564 ( 77 % ) after orthopaedic surgery , and 74 ( 23 % ) after cancer surgery ( p & lt ; 0.001 ) .
	manualset3
237991	7	421881	7	NULL	NULL	0	NULL	orthopaedic surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	At discharge , 638 ( 61 % ) patients received prescription for extended pharmacological prophylaxis : 564 ( 77 % ) after orthopaedic surgery , and 74 ( 23 % ) after cancer surgery ( p & lt ; 0.001 ) .
	manualset3
237992	8	421881	7	NULL	NULL	0	NULL	 74	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	At discharge , 638 ( 61 % ) patients received prescription for extended pharmacological prophylaxis : 564 ( 77 % ) after orthopaedic surgery , and 74 ( 23 % ) after cancer surgery ( p & lt ; 0.001 ) .
	manualset3
237993	9	421881	7	NULL	NULL	0	NULL	 23 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	At discharge , 638 ( 61 % ) patients received prescription for extended pharmacological prophylaxis : 564 ( 77 % ) after orthopaedic surgery , and 74 ( 23 % ) after cancer surgery ( p & lt ; 0.001 ) .
	manualset3
237994	10	421881	7	NULL	NULL	0	NULL	cancer surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	At discharge , 638 ( 61 % ) patients received prescription for extended pharmacological prophylaxis : 564 ( 77 % ) after orthopaedic surgery , and 74 ( 23 % ) after cancer surgery ( p & lt ; 0.001 ) .
	manualset3
237995	11	421881	7	NULL	NULL	0	NULL	p & lt ; 0.001	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	At discharge , 638 ( 61 % ) patients received prescription for extended pharmacological prophylaxis : 564 ( 77 % ) after orthopaedic surgery , and 74 ( 23 % ) after cancer surgery ( p & lt ; 0.001 ) .
	manualset3
237996	1	421882	7	NULL	NULL	0	NULL	SBP	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	SBP in 9-year-old children is independently associated with fat mass and lean mass and , to a lesser extent , trunk fat in girls .
	manualset3
237997	2	421882	7	NULL	NULL	0	NULL	9-year-old children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	SBP in 9-year-old children is independently associated with fat mass and lean mass and , to a lesser extent , trunk fat in girls .
	manualset3
237998	3	421882	7	NULL	NULL	0	NULL	fat mass	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	SBP in 9-year-old children is independently associated with fat mass and lean mass and , to a lesser extent , trunk fat in girls .
	manualset3
237999	4	421882	7	NULL	NULL	0	NULL	lean mass	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	SBP in 9-year-old children is independently associated with fat mass and lean mass and , to a lesser extent , trunk fat in girls .
	manualset3
238000	5	421882	7	NULL	NULL	0	NULL	trunk fat 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	SBP in 9-year-old children is independently associated with fat mass and lean mass and , to a lesser extent , trunk fat in girls .
	manualset3
238001	6	421882	7	NULL	NULL	0	NULL	girls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	SBP in 9-year-old children is independently associated with fat mass and lean mass and , to a lesser extent , trunk fat in girls .
	manualset3
238002	1	421883	7	NULL	NULL	0	NULL	Late clinical testing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Late clinical testing of cognition enhancers : demonstration of efficacy .
	manualset3
238003	2	421883	7	NULL	NULL	0	NULL	cognition enhancers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Late clinical testing of cognition enhancers : demonstration of efficacy .
	manualset3
238004	3	421883	7	NULL	NULL	0	NULL	demonstration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Late clinical testing of cognition enhancers : demonstration of efficacy .
	manualset3
238005	1	421884	7	NULL	NULL	0	NULL	Subclavian steal phenomenon	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Subclavian steal phenomenon associated with stress polycythemia .
	manualset3
238006	2	421884	7	NULL	NULL	0	NULL	stress polycythemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Subclavian steal phenomenon associated with stress polycythemia .
	manualset3
238008	1	421885	7	NULL	NULL	0	NULL	Thermodynamic potentials	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermodynamic potentials were determined for oleate and arachidonate binding to a subset of the FABP and retinoid binding proteins .
	manualset3
238009	2	421885	7	NULL	NULL	NULL	NULL	oleate binding	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Thermodynamic potentials were determined for oleate and arachidonate binding to a subset of the FABP and retinoid binding proteins .
	manualset3
238010	3	421885	7	NULL	NULL	NULL	NULL	arachidonate binding	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Thermodynamic potentials were determined for oleate and arachidonate binding to a subset of the FABP and retinoid binding proteins .
	manualset3
238011	4	421885	7	NULL	NULL	0	NULL	subset 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermodynamic potentials were determined for oleate and arachidonate binding to a subset of the FABP and retinoid binding proteins .
	manualset3
238012	5	421885	7	NULL	NULL	0	NULL	FABP 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermodynamic potentials were determined for oleate and arachidonate binding to a subset of the FABP and retinoid binding proteins .
	manualset3
238013	6	421885	7	NULL	NULL	0	NULL	retinoid binding proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermodynamic potentials were determined for oleate and arachidonate binding to a subset of the FABP and retinoid binding proteins .
	manualset3
238014	1	421886	7	NULL	NULL	0	NULL	Heparin-binding hemagglutinin HBHA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Heparin-binding hemagglutinin HBHA from Mycobacterium tuberculosis affects actin polymerisation .
	manualset3
238015	2	421886	7	NULL	NULL	0	NULL	Mycobacterium tuberculosis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Heparin-binding hemagglutinin HBHA from Mycobacterium tuberculosis affects actin polymerisation .
	manualset3
238016	3	421886	7	NULL	NULL	0	NULL	actin polymerisation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Heparin-binding hemagglutinin HBHA from Mycobacterium tuberculosis affects actin polymerisation .
	manualset3
238380	1	421887	7	NULL	NULL	NULL	NULL	practical synthetic method	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An efficient and practical synthetic method for the functionalized 2-amino hydropyridines and 2-pyridinones was successfully developed via the domino reactions of arylamines , methyl propiolate , aromatic aldehydes and the substituted acetonitriles with triethylamine as base catalyst .
	manualset3
238381	2	421887	7	NULL	NULL	0	NULL	 2-amino hydropyridines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An efficient and practical synthetic method for the functionalized 2-amino hydropyridines and 2-pyridinones was successfully developed via the domino reactions of arylamines , methyl propiolate , aromatic aldehydes and the substituted acetonitriles with triethylamine as base catalyst .
	manualset3
238382	3	421887	7	NULL	NULL	0	NULL	2-pyridinones	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An efficient and practical synthetic method for the functionalized 2-amino hydropyridines and 2-pyridinones was successfully developed via the domino reactions of arylamines , methyl propiolate , aromatic aldehydes and the substituted acetonitriles with triethylamine as base catalyst .
	manualset3
238383	4	421887	7	NULL	NULL	0	NULL	 domino reactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An efficient and practical synthetic method for the functionalized 2-amino hydropyridines and 2-pyridinones was successfully developed via the domino reactions of arylamines , methyl propiolate , aromatic aldehydes and the substituted acetonitriles with triethylamine as base catalyst .
	manualset3
238384	5	421887	7	NULL	NULL	0	NULL	arylamines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An efficient and practical synthetic method for the functionalized 2-amino hydropyridines and 2-pyridinones was successfully developed via the domino reactions of arylamines , methyl propiolate , aromatic aldehydes and the substituted acetonitriles with triethylamine as base catalyst .
	manualset3
238385	6	421887	7	NULL	NULL	0	NULL	methyl propiolate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An efficient and practical synthetic method for the functionalized 2-amino hydropyridines and 2-pyridinones was successfully developed via the domino reactions of arylamines , methyl propiolate , aromatic aldehydes and the substituted acetonitriles with triethylamine as base catalyst .
	manualset3
238386	7	421887	7	NULL	NULL	0	NULL	aromatic aldehydes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An efficient and practical synthetic method for the functionalized 2-amino hydropyridines and 2-pyridinones was successfully developed via the domino reactions of arylamines , methyl propiolate , aromatic aldehydes and the substituted acetonitriles with triethylamine as base catalyst .
	manualset3
238387	8	421887	7	NULL	NULL	0	NULL	substituted acetonitriles	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An efficient and practical synthetic method for the functionalized 2-amino hydropyridines and 2-pyridinones was successfully developed via the domino reactions of arylamines , methyl propiolate , aromatic aldehydes and the substituted acetonitriles with triethylamine as base catalyst .
	manualset3
238388	9	421887	7	NULL	NULL	0	NULL	 triethylamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An efficient and practical synthetic method for the functionalized 2-amino hydropyridines and 2-pyridinones was successfully developed via the domino reactions of arylamines , methyl propiolate , aromatic aldehydes and the substituted acetonitriles with triethylamine as base catalyst .
	manualset3
238389	10	421887	7	NULL	NULL	0	NULL	 base catalyst	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An efficient and practical synthetic method for the functionalized 2-amino hydropyridines and 2-pyridinones was successfully developed via the domino reactions of arylamines , methyl propiolate , aromatic aldehydes and the substituted acetonitriles with triethylamine as base catalyst .
	manualset3
238390	1	421888	7	NULL	NULL	0	NULL	Two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two of 7 growth-inhibitory antibodies also block the binding and function of the gp30 and p75 c-erbB-2 ligands .
	manualset3
238391	2	421888	7	NULL	NULL	0	NULL	7 growth-inhibitory antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two of 7 growth-inhibitory antibodies also block the binding and function of the gp30 and p75 c-erbB-2 ligands .
	manualset3
238392	3	421888	7	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two of 7 growth-inhibitory antibodies also block the binding and function of the gp30 and p75 c-erbB-2 ligands .
	manualset3
238393	4	421888	7	NULL	NULL	0	NULL	function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two of 7 growth-inhibitory antibodies also block the binding and function of the gp30 and p75 c-erbB-2 ligands .
	manualset3
238394	5	421888	7	NULL	NULL	0	NULL	 gp30	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Two of 7 growth-inhibitory antibodies also block the binding and function of the gp30 and p75 c-erbB-2 ligands .
	manualset3
238395	6	421888	7	NULL	NULL	0	NULL	 p75 c-erbB-2 ligands	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two of 7 growth-inhibitory antibodies also block the binding and function of the gp30 and p75 c-erbB-2 ligands .
	manualset3
238396	1	421889	7	NULL	NULL	0	NULL	situation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The situation at the beginning of the 21st century ) .
	manualset3
238397	2	421889	7	NULL	NULL	0	NULL	beginning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The situation at the beginning of the 21st century ) .
	manualset3
238398	3	421889	7	NULL	NULL	0	NULL	21st century	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	The situation at the beginning of the 21st century ) .
	manualset3
238426	1	421890	7	NULL	NULL	0	NULL	Jak2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , Jak2 can not be a sole therapeutic target to treat the established disease .
	manualset3
238429	2	421890	7	NULL	NULL	0	NULL	therapeutic target 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , Jak2 can not be a sole therapeutic target to treat the established disease .
	manualset3
238430	3	421890	7	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , Jak2 can not be a sole therapeutic target to treat the established disease .
	manualset3
238445	1	421891	7	NULL	NULL	0	NULL	Argininamide binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Argininamide binding arrests global motions in HIV-1 TAR RNA : comparison with Mg2 + - induced conformational stabilization .
	manualset3
238447	2	421891	7	NULL	NULL	0	NULL	global motions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Argininamide binding arrests global motions in HIV-1 TAR RNA : comparison with Mg2 + - induced conformational stabilization .
	manualset3
238448	3	421891	7	NULL	NULL	0	NULL	HIV-1 TAR RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Argininamide binding arrests global motions in HIV-1 TAR RNA : comparison with Mg2 + - induced conformational stabilization .
	manualset3
238449	4	421891	7	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Argininamide binding arrests global motions in HIV-1 TAR RNA : comparison with Mg2 + - induced conformational stabilization .
	manualset3
238451	5	421891	7	NULL	NULL	0	NULL	Mg2 + - induced conformational stabilization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Argininamide binding arrests global motions in HIV-1 TAR RNA : comparison with Mg2 + - induced conformational stabilization .
	manualset3
238461	1	421892	7	NULL	NULL	0	NULL	enantioselective N-specific reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An enantioselective N-specific reaction of nitrosobenzene with unmodified aldehydes was successfully achieved catalyzed first by a variety of primary amine-based organocatalysts with higher yield and enantioselectivity .
	manualset3
238462	2	421892	7	NULL	NULL	0	NULL	nitrosobenzene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An enantioselective N-specific reaction of nitrosobenzene with unmodified aldehydes was successfully achieved catalyzed first by a variety of primary amine-based organocatalysts with higher yield and enantioselectivity .
	manualset3
238463	3	421892	7	NULL	NULL	0	NULL	unmodified aldehydes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An enantioselective N-specific reaction of nitrosobenzene with unmodified aldehydes was successfully achieved catalyzed first by a variety of primary amine-based organocatalysts with higher yield and enantioselectivity .
	manualset3
238465	4	421892	7	NULL	NULL	0	NULL	primary amine-based organocatalysts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An enantioselective N-specific reaction of nitrosobenzene with unmodified aldehydes was successfully achieved catalyzed first by a variety of primary amine-based organocatalysts with higher yield and enantioselectivity .
	manualset3
238466	5	421892	7	NULL	NULL	0	NULL	higher yield	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An enantioselective N-specific reaction of nitrosobenzene with unmodified aldehydes was successfully achieved catalyzed first by a variety of primary amine-based organocatalysts with higher yield and enantioselectivity .
	manualset3
238467	6	421892	7	NULL	NULL	0	NULL	enantioselectivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An enantioselective N-specific reaction of nitrosobenzene with unmodified aldehydes was successfully achieved catalyzed first by a variety of primary amine-based organocatalysts with higher yield and enantioselectivity .
	manualset3
238476	1	421893	7	NULL	NULL	0	NULL	key roles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The key roles of imaging in inflammatory breast cancer using mammography , sonography , magnetic resonance imaging , and positron emission tomography/computed tomography to facilitate image-guided biopsy for biomarker evaluation , delineate disease extent , diagnose distant metastases , and monitor response to therapy are described in this article .
	manualset3
238477	2	421893	7	NULL	NULL	NULL	NULL	imaging	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The key roles of imaging in inflammatory breast cancer using mammography , sonography , magnetic resonance imaging , and positron emission tomography/computed tomography to facilitate image-guided biopsy for biomarker evaluation , delineate disease extent , diagnose distant metastases , and monitor response to therapy are described in this article .
	manualset3
238478	3	421893	7	NULL	NULL	0	NULL	inflammatory breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The key roles of imaging in inflammatory breast cancer using mammography , sonography , magnetic resonance imaging , and positron emission tomography/computed tomography to facilitate image-guided biopsy for biomarker evaluation , delineate disease extent , diagnose distant metastases , and monitor response to therapy are described in this article .
	manualset3
238484	4	421893	7	NULL	NULL	0	NULL	mammography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The key roles of imaging in inflammatory breast cancer using mammography , sonography , magnetic resonance imaging , and positron emission tomography/computed tomography to facilitate image-guided biopsy for biomarker evaluation , delineate disease extent , diagnose distant metastases , and monitor response to therapy are described in this article .
	manualset3
238486	5	421893	7	NULL	NULL	0	NULL	sonography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The key roles of imaging in inflammatory breast cancer using mammography , sonography , magnetic resonance imaging , and positron emission tomography/computed tomography to facilitate image-guided biopsy for biomarker evaluation , delineate disease extent , diagnose distant metastases , and monitor response to therapy are described in this article .
	manualset3
238487	6	421893	7	NULL	NULL	0	NULL	magnetic resonance imaging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The key roles of imaging in inflammatory breast cancer using mammography , sonography , magnetic resonance imaging , and positron emission tomography/computed tomography to facilitate image-guided biopsy for biomarker evaluation , delineate disease extent , diagnose distant metastases , and monitor response to therapy are described in this article .
	manualset3
238489	7	421893	7	NULL	NULL	0	NULL	positron emission tomography/computed tomography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The key roles of imaging in inflammatory breast cancer using mammography , sonography , magnetic resonance imaging , and positron emission tomography/computed tomography to facilitate image-guided biopsy for biomarker evaluation , delineate disease extent , diagnose distant metastases , and monitor response to therapy are described in this article .
	manualset3
238492	8	421893	7	NULL	NULL	0	NULL	image-guided biopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The key roles of imaging in inflammatory breast cancer using mammography , sonography , magnetic resonance imaging , and positron emission tomography/computed tomography to facilitate image-guided biopsy for biomarker evaluation , delineate disease extent , diagnose distant metastases , and monitor response to therapy are described in this article .
	manualset3
238493	9	421893	7	NULL	NULL	0	NULL	biomarker evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The key roles of imaging in inflammatory breast cancer using mammography , sonography , magnetic resonance imaging , and positron emission tomography/computed tomography to facilitate image-guided biopsy for biomarker evaluation , delineate disease extent , diagnose distant metastases , and monitor response to therapy are described in this article .
	manualset3
238495	10	421893	7	NULL	NULL	0	NULL	distant metastases	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The key roles of imaging in inflammatory breast cancer using mammography , sonography , magnetic resonance imaging , and positron emission tomography/computed tomography to facilitate image-guided biopsy for biomarker evaluation , delineate disease extent , diagnose distant metastases , and monitor response to therapy are described in this article .
	manualset3
238497	11	421893	7	NULL	NULL	0	NULL	 therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The key roles of imaging in inflammatory breast cancer using mammography , sonography , magnetic resonance imaging , and positron emission tomography/computed tomography to facilitate image-guided biopsy for biomarker evaluation , delineate disease extent , diagnose distant metastases , and monitor response to therapy are described in this article .
	manualset3
238498	12	421893	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The key roles of imaging in inflammatory breast cancer using mammography , sonography , magnetic resonance imaging , and positron emission tomography/computed tomography to facilitate image-guided biopsy for biomarker evaluation , delineate disease extent , diagnose distant metastases , and monitor response to therapy are described in this article .
	manualset3
242880	13	421893	7	NULL	NULL	0	NULL	disease extent	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The key roles of imaging in inflammatory breast cancer using mammography , sonography , magnetic resonance imaging , and positron emission tomography/computed tomography to facilitate image-guided biopsy for biomarker evaluation , delineate disease extent , diagnose distant metastases , and monitor response to therapy are described in this article .
	manualset3
243954	14	421893	7	NULL	NULL	0	NULL	response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The key roles of imaging in inflammatory breast cancer using mammography , sonography , magnetic resonance imaging , and positron emission tomography/computed tomography to facilitate image-guided biopsy for biomarker evaluation , delineate disease extent , diagnose distant metastases , and monitor response to therapy are described in this article .
	manualset3
238544	1	421894	7	NULL	NULL	0	NULL	Monozygotic twin correlations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Monozygotic twin correlations were consistently higher than twice the dizygotic twin correlations for all 7 scales , suggesting pervasive influences of nonadditive genetic effects on personality traits in the South Korean population .
	manualset3
238547	2	421894	7	NULL	NULL	0	NULL	dizygotic twin correlations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Monozygotic twin correlations were consistently higher than twice the dizygotic twin correlations for all 7 scales , suggesting pervasive influences of nonadditive genetic effects on personality traits in the South Korean population .
	manualset3
238550	3	421894	7	NULL	NULL	0	NULL	7 scales	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Monozygotic twin correlations were consistently higher than twice the dizygotic twin correlations for all 7 scales , suggesting pervasive influences of nonadditive genetic effects on personality traits in the South Korean population .
	manualset3
238552	4	421894	7	NULL	NULL	0	NULL	nonadditive genetic effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Monozygotic twin correlations were consistently higher than twice the dizygotic twin correlations for all 7 scales , suggesting pervasive influences of nonadditive genetic effects on personality traits in the South Korean population .
	manualset3
238556	5	421894	7	NULL	NULL	0	NULL	personality traits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Monozygotic twin correlations were consistently higher than twice the dizygotic twin correlations for all 7 scales , suggesting pervasive influences of nonadditive genetic effects on personality traits in the South Korean population .
	manualset3
238557	6	421894	7	NULL	NULL	0	NULL	South Korean population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Monozygotic twin correlations were consistently higher than twice the dizygotic twin correlations for all 7 scales , suggesting pervasive influences of nonadditive genetic effects on personality traits in the South Korean population .
	manualset3
238569	1	421895	7	NULL	NULL	0	NULL	 efficient automated algorithm	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	An efficient automated algorithm to detect ocular surface temperature on sequence of thermograms using snake and target tracing function .
	manualset3
238571	2	421895	7	NULL	NULL	0	NULL	ocular surface temperature	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An efficient automated algorithm to detect ocular surface temperature on sequence of thermograms using snake and target tracing function .
	manualset3
238572	3	421895	7	NULL	NULL	0	NULL	sequence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An efficient automated algorithm to detect ocular surface temperature on sequence of thermograms using snake and target tracing function .
	manualset3
238578	4	421895	7	NULL	NULL	0	NULL	thermograms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An efficient automated algorithm to detect ocular surface temperature on sequence of thermograms using snake and target tracing function .
	manualset3
238580	5	421895	7	NULL	NULL	0	NULL	snake function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An efficient automated algorithm to detect ocular surface temperature on sequence of thermograms using snake and target tracing function .
	manualset3
238581	6	421895	7	NULL	NULL	0	NULL	target tracing function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An efficient automated algorithm to detect ocular surface temperature on sequence of thermograms using snake and target tracing function .
	manualset3
238679	1	421896	7	NULL	NULL	0	NULL	Intrcranial gliomata	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Intrcranial gliomata : some clinical , radiological and therapeutic aspects of 298 cases .
	manualset3
238680	2	421896	7	NULL	NULL	0	NULL	therapeutic aspects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Intrcranial gliomata : some clinical , radiological and therapeutic aspects of 298 cases .
	manualset3
238681	3	421896	7	NULL	NULL	0	NULL	298 cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intrcranial gliomata : some clinical , radiological and therapeutic aspects of 298 cases .
	manualset3
238690	1	421897	7	NULL	NULL	0	NULL	HPGDS	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	HPGDS was expressed in the epithelium of immature and cycling mice but not in the oviducts of estrogen receptor knockouts .
	manualset3
238692	2	421897	7	NULL	NULL	0	NULL	epithelium	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	HPGDS was expressed in the epithelium of immature and cycling mice but not in the oviducts of estrogen receptor knockouts .
	manualset3
238694	3	421897	7	NULL	NULL	0	NULL	immature mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	HPGDS was expressed in the epithelium of immature and cycling mice but not in the oviducts of estrogen receptor knockouts .
	manualset3
238695	4	421897	7	NULL	NULL	0	NULL	cycling mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	HPGDS was expressed in the epithelium of immature and cycling mice but not in the oviducts of estrogen receptor knockouts .
	manualset3
238698	5	421897	7	NULL	NULL	0	NULL	oviducts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	HPGDS was expressed in the epithelium of immature and cycling mice but not in the oviducts of estrogen receptor knockouts .
	manualset3
238699	6	421897	7	NULL	NULL	0	NULL	estrogen receptor knockouts	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	HPGDS was expressed in the epithelium of immature and cycling mice but not in the oviducts of estrogen receptor knockouts .
	manualset3
238701	1	421898	7	NULL	NULL	0	NULL	coil-to-helix transition 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We have studied the coil-to-helix transition of the DNA oligomer d ( C4A4T4C4 ) , using circular dichroism measurements to monitor the formation of A.T base pairs within the central self-complementary A4T4 region and the formation of protonated C. C + base pairs at the ends of the oligomer .
	manualset3
238703	2	421898	7	NULL	NULL	0	NULL	DNA oligomer d ( C4A4T4C4 ) 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	We have studied the coil-to-helix transition of the DNA oligomer d ( C4A4T4C4 ) , using circular dichroism measurements to monitor the formation of A.T base pairs within the central self-complementary A4T4 region and the formation of protonated C. C + base pairs at the ends of the oligomer .
	manualset3
238704	3	421898	7	NULL	NULL	0	NULL	circular dichroism measurements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We have studied the coil-to-helix transition of the DNA oligomer d ( C4A4T4C4 ) , using circular dichroism measurements to monitor the formation of A.T base pairs within the central self-complementary A4T4 region and the formation of protonated C. C + base pairs at the ends of the oligomer .
	manualset3
238705	4	421898	7	NULL	NULL	0	NULL	formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We have studied the coil-to-helix transition of the DNA oligomer d ( C4A4T4C4 ) , using circular dichroism measurements to monitor the formation of A.T base pairs within the central self-complementary A4T4 region and the formation of protonated C. C + base pairs at the ends of the oligomer .
	manualset3
238709	5	421898	7	NULL	NULL	0	NULL	A.T base pairs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	We have studied the coil-to-helix transition of the DNA oligomer d ( C4A4T4C4 ) , using circular dichroism measurements to monitor the formation of A.T base pairs within the central self-complementary A4T4 region and the formation of protonated C. C + base pairs at the ends of the oligomer .
	manualset3
238710	6	421898	7	NULL	NULL	0	NULL	central self-complementary A4T4 region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	We have studied the coil-to-helix transition of the DNA oligomer d ( C4A4T4C4 ) , using circular dichroism measurements to monitor the formation of A.T base pairs within the central self-complementary A4T4 region and the formation of protonated C. C + base pairs at the ends of the oligomer .
	manualset3
238715	7	421898	7	NULL	NULL	0	NULL	formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We have studied the coil-to-helix transition of the DNA oligomer d ( C4A4T4C4 ) , using circular dichroism measurements to monitor the formation of A.T base pairs within the central self-complementary A4T4 region and the formation of protonated C. C + base pairs at the ends of the oligomer .
	manualset3
238716	8	421898	7	NULL	NULL	0	NULL	 protonated C. C + base pairs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	We have studied the coil-to-helix transition of the DNA oligomer d ( C4A4T4C4 ) , using circular dichroism measurements to monitor the formation of A.T base pairs within the central self-complementary A4T4 region and the formation of protonated C. C + base pairs at the ends of the oligomer .
	manualset3
238717	9	421898	7	NULL	NULL	0	NULL	ends	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	We have studied the coil-to-helix transition of the DNA oligomer d ( C4A4T4C4 ) , using circular dichroism measurements to monitor the formation of A.T base pairs within the central self-complementary A4T4 region and the formation of protonated C. C + base pairs at the ends of the oligomer .
	manualset3
238718	10	421898	7	NULL	NULL	0	NULL	 oligomer 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	We have studied the coil-to-helix transition of the DNA oligomer d ( C4A4T4C4 ) , using circular dichroism measurements to monitor the formation of A.T base pairs within the central self-complementary A4T4 region and the formation of protonated C. C + base pairs at the ends of the oligomer .
	manualset3
238791	1	421899	7	NULL	NULL	0	NULL	Synaptic potentials	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Synaptic potentials were studied using extracellular , intracellular and single-electrode voltage clamp techniques .
	manualset3
238792	2	421899	7	NULL	NULL	0	NULL	extracellular  voltage clamp techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Synaptic potentials were studied using extracellular , intracellular and single-electrode voltage clamp techniques .
	manualset3
238793	3	421899	7	NULL	NULL	0	NULL	intracellular voltage clamp techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Synaptic potentials were studied using extracellular , intracellular and single-electrode voltage clamp techniques .
	manualset3
238794	4	421899	7	NULL	NULL	0	NULL	single-electrode voltage clamp techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Synaptic potentials were studied using extracellular , intracellular and single-electrode voltage clamp techniques .
	manualset3
238795	1	421900	7	NULL	NULL	0	NULL	Examination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Examination related to revised test method for determination of formaldehyde , regulated by the law for the control of household products containing harmful substances ) .
	manualset3
238796	2	421900	7	NULL	NULL	0	NULL	revised test method 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Examination related to revised test method for determination of formaldehyde , regulated by the law for the control of household products containing harmful substances ) .
	manualset3
238797	3	421900	7	NULL	NULL	0	NULL	determination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Examination related to revised test method for determination of formaldehyde , regulated by the law for the control of household products containing harmful substances ) .
	manualset3
238798	4	421900	7	NULL	NULL	0	NULL	formaldehyde	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Examination related to revised test method for determination of formaldehyde , regulated by the law for the control of household products containing harmful substances ) .
	manualset3
238799	5	421900	7	NULL	NULL	0	NULL	law	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Examination related to revised test method for determination of formaldehyde , regulated by the law for the control of household products containing harmful substances ) .
	manualset3
238800	6	421900	7	NULL	NULL	0	NULL	control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Examination related to revised test method for determination of formaldehyde , regulated by the law for the control of household products containing harmful substances ) .
	manualset3
238802	7	421900	7	NULL	NULL	0	NULL	household products	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Examination related to revised test method for determination of formaldehyde , regulated by the law for the control of household products containing harmful substances ) .
	manualset3
238803	8	421900	7	NULL	NULL	0	NULL	harmful substances	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Examination related to revised test method for determination of formaldehyde , regulated by the law for the control of household products containing harmful substances ) .
	manualset3
238805	1	421901	7	NULL	NULL	0	NULL	Herpes simplex viruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Herpes simplex viruses establish latency in the nuclei of neuronal cells and may reactivate , with or without symptoms , throughout the host 's lifetime .
	manualset3
238806	2	421901	7	NULL	NULL	0	NULL	 nuclei 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Herpes simplex viruses establish latency in the nuclei of neuronal cells and may reactivate , with or without symptoms , throughout the host 's lifetime .
	manualset3
238807	3	421901	7	NULL	NULL	0	NULL	neuronal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Herpes simplex viruses establish latency in the nuclei of neuronal cells and may reactivate , with or without symptoms , throughout the host 's lifetime .
	manualset3
238808	4	421901	7	NULL	NULL	0	NULL	symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Herpes simplex viruses establish latency in the nuclei of neuronal cells and may reactivate , with or without symptoms , throughout the host 's lifetime .
	manualset3
238809	5	421901	7	NULL	NULL	NULL	NULL	host 's lifetime	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Herpes simplex viruses establish latency in the nuclei of neuronal cells and may reactivate , with or without symptoms , throughout the host 's lifetime .
	manualset3
238813	1	421902	7	NULL	NULL	0	NULL	FM19	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	FM19 , which completely inhibits threshold gamma-thrombin-induced platelet aggregation at a concentration of 16 + / - 4 microm , represents an important lead compound in the development of inhibitors of thrombin-mediated platelet aggregation for treatment of ACS .
	manualset3
238814	2	421902	7	NULL	NULL	0	NULL	gamma-thrombin-induced platelet aggregation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	FM19 , which completely inhibits threshold gamma-thrombin-induced platelet aggregation at a concentration of 16 + / - 4 microm , represents an important lead compound in the development of inhibitors of thrombin-mediated platelet aggregation for treatment of ACS .
	manualset3
238815	3	421902	7	NULL	NULL	0	NULL	concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	FM19 , which completely inhibits threshold gamma-thrombin-induced platelet aggregation at a concentration of 16 + / - 4 microm , represents an important lead compound in the development of inhibitors of thrombin-mediated platelet aggregation for treatment of ACS .
	manualset3
238816	4	421902	7	NULL	NULL	0	NULL	16 + / - 4 microm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	FM19 , which completely inhibits threshold gamma-thrombin-induced platelet aggregation at a concentration of 16 + / - 4 microm , represents an important lead compound in the development of inhibitors of thrombin-mediated platelet aggregation for treatment of ACS .
	manualset3
238817	5	421902	7	NULL	NULL	0	NULL	lead compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	FM19 , which completely inhibits threshold gamma-thrombin-induced platelet aggregation at a concentration of 16 + / - 4 microm , represents an important lead compound in the development of inhibitors of thrombin-mediated platelet aggregation for treatment of ACS .
	manualset3
238818	6	421902	7	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	FM19 , which completely inhibits threshold gamma-thrombin-induced platelet aggregation at a concentration of 16 + / - 4 microm , represents an important lead compound in the development of inhibitors of thrombin-mediated platelet aggregation for treatment of ACS .
	manualset3
238819	7	421902	7	NULL	NULL	0	NULL	inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	FM19 , which completely inhibits threshold gamma-thrombin-induced platelet aggregation at a concentration of 16 + / - 4 microm , represents an important lead compound in the development of inhibitors of thrombin-mediated platelet aggregation for treatment of ACS .
	manualset3
238820	8	421902	7	NULL	NULL	0	NULL	thrombin-mediated platelet aggregation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	FM19 , which completely inhibits threshold gamma-thrombin-induced platelet aggregation at a concentration of 16 + / - 4 microm , represents an important lead compound in the development of inhibitors of thrombin-mediated platelet aggregation for treatment of ACS .
	manualset3
238822	9	421902	7	NULL	NULL	0	NULL	 treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	FM19 , which completely inhibits threshold gamma-thrombin-induced platelet aggregation at a concentration of 16 + / - 4 microm , represents an important lead compound in the development of inhibitors of thrombin-mediated platelet aggregation for treatment of ACS .
	manualset3
238823	10	421902	7	NULL	NULL	0	NULL	ACS 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	FM19 , which completely inhibits threshold gamma-thrombin-induced platelet aggregation at a concentration of 16 + / - 4 microm , represents an important lead compound in the development of inhibitors of thrombin-mediated platelet aggregation for treatment of ACS .
	manualset3
238825	1	421903	7	NULL	NULL	0	NULL	Antioxidants 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Antioxidants , such as alpha-tocopherol and all-trans-retinol acetate , inhibited the isomerization process .
	manualset3
238827	2	421903	7	NULL	NULL	0	NULL	alpha-tocopherol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Antioxidants , such as alpha-tocopherol and all-trans-retinol acetate , inhibited the isomerization process .
	manualset3
238828	3	421903	7	NULL	NULL	0	NULL	all-trans-retinol acetate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Antioxidants , such as alpha-tocopherol and all-trans-retinol acetate , inhibited the isomerization process .
	manualset3
238829	4	421903	7	NULL	NULL	0	NULL	isomerization process	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antioxidants , such as alpha-tocopherol and all-trans-retinol acetate , inhibited the isomerization process .
	manualset3
238830	1	421904	7	NULL	NULL	0	NULL	efficient expression/secretion vector	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	An efficient expression/secretion vector , designated pM2Veg , was constructed for extracellular production of heterologous proteins in Bacillus subtilis .
	manualset3
238831	2	421904	7	NULL	NULL	0	NULL	pM2Veg	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	An efficient expression/secretion vector , designated pM2Veg , was constructed for extracellular production of heterologous proteins in Bacillus subtilis .
	manualset3
238832	3	421904	7	NULL	NULL	0	NULL	extracellular production 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An efficient expression/secretion vector , designated pM2Veg , was constructed for extracellular production of heterologous proteins in Bacillus subtilis .
	manualset3
238833	4	421904	7	NULL	NULL	0	NULL	heterologous proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	An efficient expression/secretion vector , designated pM2Veg , was constructed for extracellular production of heterologous proteins in Bacillus subtilis .
	manualset3
238834	5	421904	7	NULL	NULL	0	NULL	Bacillus subtilis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	An efficient expression/secretion vector , designated pM2Veg , was constructed for extracellular production of heterologous proteins in Bacillus subtilis .
	manualset3
238837	1	421905	7	NULL	NULL	0	NULL	19 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , we studied 19 patients with simultaneous high-fidelity micromanometer LV and fluid brachial artery ( Ba ) pressure recordings , CINE , and RNA under control conditions and during methoxamine and nitroprusside infusions .
	manualset3
238841	2	421905	7	NULL	NULL	0	NULL	high-fidelity micromanometer LV	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , we studied 19 patients with simultaneous high-fidelity micromanometer LV and fluid brachial artery ( Ba ) pressure recordings , CINE , and RNA under control conditions and during methoxamine and nitroprusside infusions .
	manualset3
238842	3	421905	7	NULL	NULL	0	NULL	luid brachial artery ( Ba ) pressure recordings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , we studied 19 patients with simultaneous high-fidelity micromanometer LV and fluid brachial artery ( Ba ) pressure recordings , CINE , and RNA under control conditions and during methoxamine and nitroprusside infusions .
	manualset3
238843	4	421905	7	NULL	NULL	0	NULL	CINE	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , we studied 19 patients with simultaneous high-fidelity micromanometer LV and fluid brachial artery ( Ba ) pressure recordings , CINE , and RNA under control conditions and during methoxamine and nitroprusside infusions .
	manualset3
238844	5	421905	7	NULL	NULL	0	NULL	RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , we studied 19 patients with simultaneous high-fidelity micromanometer LV and fluid brachial artery ( Ba ) pressure recordings , CINE , and RNA under control conditions and during methoxamine and nitroprusside infusions .
	manualset3
238845	6	421905	7	NULL	NULL	0	NULL	control conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , we studied 19 patients with simultaneous high-fidelity micromanometer LV and fluid brachial artery ( Ba ) pressure recordings , CINE , and RNA under control conditions and during methoxamine and nitroprusside infusions .
	manualset3
238846	7	421905	7	NULL	NULL	0	NULL	methoxamine infusions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , we studied 19 patients with simultaneous high-fidelity micromanometer LV and fluid brachial artery ( Ba ) pressure recordings , CINE , and RNA under control conditions and during methoxamine and nitroprusside infusions .
	manualset3
238847	8	421905	7	NULL	NULL	0	NULL	nitroprusside infusions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , we studied 19 patients with simultaneous high-fidelity micromanometer LV and fluid brachial artery ( Ba ) pressure recordings , CINE , and RNA under control conditions and during methoxamine and nitroprusside infusions .
	manualset3
238848	1	421906	7	NULL	NULL	0	NULL	adolescents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , among adolescents , more frequent alcohol use was associated with lower follow-up rates .
	manualset3
238849	2	421906	7	NULL	NULL	0	NULL	alcohol use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , among adolescents , more frequent alcohol use was associated with lower follow-up rates .
	manualset3
238850	3	421906	7	NULL	NULL	0	NULL	lower follow-up rates	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Additionally , among adolescents , more frequent alcohol use was associated with lower follow-up rates .
	manualset3
238851	1	421907	7	NULL	NULL	0	NULL	Langmuir equation	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the Langmuir equation , the maximum uptake capacities ( q ( m ) ) for MB , RB and BM were 869.6 , 267.4 and 719.4 mg g ( -1 ) , which were 17 - , 11 - and 12-fold of that obtained on the unmodified biomass , respectively .
	manualset3
238852	2	421907	7	NULL	NULL	0	NULL	maximum uptake capacities ( q ( m ) )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the Langmuir equation , the maximum uptake capacities ( q ( m ) ) for MB , RB and BM were 869.6 , 267.4 and 719.4 mg g ( -1 ) , which were 17 - , 11 - and 12-fold of that obtained on the unmodified biomass , respectively .
	manualset3
238853	3	421907	7	NULL	NULL	0	NULL	MB	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the Langmuir equation , the maximum uptake capacities ( q ( m ) ) for MB , RB and BM were 869.6 , 267.4 and 719.4 mg g ( -1 ) , which were 17 - , 11 - and 12-fold of that obtained on the unmodified biomass , respectively .
	manualset3
238854	4	421907	7	NULL	NULL	0	NULL	RB	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the Langmuir equation , the maximum uptake capacities ( q ( m ) ) for MB , RB and BM were 869.6 , 267.4 and 719.4 mg g ( -1 ) , which were 17 - , 11 - and 12-fold of that obtained on the unmodified biomass , respectively .
	manualset3
238855	5	421907	7	NULL	NULL	0	NULL	BM	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the Langmuir equation , the maximum uptake capacities ( q ( m ) ) for MB , RB and BM were 869.6 , 267.4 and 719.4 mg g ( -1 ) , which were 17 - , 11 - and 12-fold of that obtained on the unmodified biomass , respectively .
	manualset3
238856	6	421907	7	NULL	NULL	0	NULL	 869.6 mg g ( -1 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the Langmuir equation , the maximum uptake capacities ( q ( m ) ) for MB , RB and BM were 869.6 , 267.4 and 719.4 mg g ( -1 ) , which were 17 - , 11 - and 12-fold of that obtained on the unmodified biomass , respectively .
	manualset3
238857	7	421907	7	NULL	NULL	0	NULL	 267.4 mg g ( -1 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the Langmuir equation , the maximum uptake capacities ( q ( m ) ) for MB , RB and BM were 869.6 , 267.4 and 719.4 mg g ( -1 ) , which were 17 - , 11 - and 12-fold of that obtained on the unmodified biomass , respectively .
	manualset3
238858	8	421907	7	NULL	NULL	0	NULL	719.4 mg g ( -1 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the Langmuir equation , the maximum uptake capacities ( q ( m ) ) for MB , RB and BM were 869.6 , 267.4 and 719.4 mg g ( -1 ) , which were 17 - , 11 - and 12-fold of that obtained on the unmodified biomass , respectively .
	manualset3
238859	9	421907	7	NULL	NULL	0	NULL	17 -fold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the Langmuir equation , the maximum uptake capacities ( q ( m ) ) for MB , RB and BM were 869.6 , 267.4 and 719.4 mg g ( -1 ) , which were 17 - , 11 - and 12-fold of that obtained on the unmodified biomass , respectively .
	manualset3
238860	10	421907	7	NULL	NULL	0	NULL	11 -fold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the Langmuir equation , the maximum uptake capacities ( q ( m ) ) for MB , RB and BM were 869.6 , 267.4 and 719.4 mg g ( -1 ) , which were 17 - , 11 - and 12-fold of that obtained on the unmodified biomass , respectively .
	manualset3
238861	11	421907	7	NULL	NULL	0	NULL	12-fold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	According to the Langmuir equation , the maximum uptake capacities ( q ( m ) ) for MB , RB and BM were 869.6 , 267.4 and 719.4 mg g ( -1 ) , which were 17 - , 11 - and 12-fold of that obtained on the unmodified biomass , respectively .
	manualset3
238862	12	421907	7	NULL	NULL	NULL	NULL	unmodified biomass	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	According to the Langmuir equation , the maximum uptake capacities ( q ( m ) ) for MB , RB and BM were 869.6 , 267.4 and 719.4 mg g ( -1 ) , which were 17 - , 11 - and 12-fold of that obtained on the unmodified biomass , respectively .
	manualset3
238863	1	421908	7	NULL	NULL	0	NULL	V. Kratschmer	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	First , we would like to thank V. Kratschmer for his validation of our results in the paper regarding the belief measure by using a topological approach .
	manualset3
238864	2	421908	7	NULL	NULL	0	NULL	validation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	First , we would like to thank V. Kratschmer for his validation of our results in the paper regarding the belief measure by using a topological approach .
	manualset3
238865	3	421908	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	First , we would like to thank V. Kratschmer for his validation of our results in the paper regarding the belief measure by using a topological approach .
	manualset3
238866	4	421908	7	NULL	NULL	0	NULL	 paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	First , we would like to thank V. Kratschmer for his validation of our results in the paper regarding the belief measure by using a topological approach .
	manualset3
238867	5	421908	7	NULL	NULL	0	NULL	topological approach	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	First , we would like to thank V. Kratschmer for his validation of our results in the paper regarding the belief measure by using a topological approach .
	manualset3
238868	1	421909	7	NULL	NULL	0	NULL	four novel PITX2-associated protein partners	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We identified four novel PITX2-associated protein partners Y box binding factor-1 , heterogeneous ribonucleoprotein K , nucleolin and heterogeneous nuclear ribonucleoprotein U in mass spectrometry analysis .
	manualset3
238869	2	421909	7	NULL	NULL	0	NULL	Y box binding factor-1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We identified four novel PITX2-associated protein partners Y box binding factor-1 , heterogeneous ribonucleoprotein K , nucleolin and heterogeneous nuclear ribonucleoprotein U in mass spectrometry analysis .
	manualset3
238870	3	421909	7	NULL	NULL	0	NULL	heterogeneous ribonucleoprotein K	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We identified four novel PITX2-associated protein partners Y box binding factor-1 , heterogeneous ribonucleoprotein K , nucleolin and heterogeneous nuclear ribonucleoprotein U in mass spectrometry analysis .
	manualset3
238871	4	421909	7	NULL	NULL	0	NULL	 nucleolin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We identified four novel PITX2-associated protein partners Y box binding factor-1 , heterogeneous ribonucleoprotein K , nucleolin and heterogeneous nuclear ribonucleoprotein U in mass spectrometry analysis .
	manualset3
238872	5	421909	7	NULL	NULL	0	NULL	heterogeneous nuclear ribonucleoprotein U	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We identified four novel PITX2-associated protein partners Y box binding factor-1 , heterogeneous ribonucleoprotein K , nucleolin and heterogeneous nuclear ribonucleoprotein U in mass spectrometry analysis .
	manualset3
238873	6	421909	7	NULL	NULL	0	NULL	mass spectrometry analysis .	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We identified four novel PITX2-associated protein partners Y box binding factor-1 , heterogeneous ribonucleoprotein K , nucleolin and heterogeneous nuclear ribonucleoprotein U in mass spectrometry analysis .
	manualset3
238874	1	421910	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained were compared with those provided by batch acid hydrolysis , and were similar in all instances .
	manualset3
238875	2	421910	7	NULL	NULL	0	NULL	batch acid hydrolysis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained were compared with those provided by batch acid hydrolysis , and were similar in all instances .
	manualset3
238876	1	421911	7	NULL	NULL	0	NULL	FFMP	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We conclude that the FFMP holds promise for studying personality traits in alcohol use disorders and in bringing a unifying perspective to research and clinical work in this area .
	manualset3
238877	2	421911	7	NULL	NULL	0	NULL	personality traits 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We conclude that the FFMP holds promise for studying personality traits in alcohol use disorders and in bringing a unifying perspective to research and clinical work in this area .
	manualset3
238878	3	421911	7	NULL	NULL	0	NULL	alcohol use disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We conclude that the FFMP holds promise for studying personality traits in alcohol use disorders and in bringing a unifying perspective to research and clinical work in this area .
	manualset3
238879	4	421911	7	NULL	NULL	0	NULL	 research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We conclude that the FFMP holds promise for studying personality traits in alcohol use disorders and in bringing a unifying perspective to research and clinical work in this area .
	manualset3
238880	5	421911	7	NULL	NULL	0	NULL	clinical work	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We conclude that the FFMP holds promise for studying personality traits in alcohol use disorders and in bringing a unifying perspective to research and clinical work in this area .
	manualset3
238881	6	421911	7	NULL	NULL	0	NULL	 area 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We conclude that the FFMP holds promise for studying personality traits in alcohol use disorders and in bringing a unifying perspective to research and clinical work in this area .
	manualset3
238882	1	421912	7	NULL	NULL	0	NULL	 efficient method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	An efficient method is presented for the assignment of the proton , carbon , and nitrogen resonances in the NMR spectra of isotopically labeled nucleic acids .
	manualset3
238883	2	421912	7	NULL	NULL	0	NULL	assignment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An efficient method is presented for the assignment of the proton , carbon , and nitrogen resonances in the NMR spectra of isotopically labeled nucleic acids .
	manualset3
238884	3	421912	7	NULL	NULL	NULL	NULL	 proton	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An efficient method is presented for the assignment of the proton , carbon , and nitrogen resonances in the NMR spectra of isotopically labeled nucleic acids .
	manualset3
238885	4	421912	7	NULL	NULL	0	NULL	carbon	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	An efficient method is presented for the assignment of the proton , carbon , and nitrogen resonances in the NMR spectra of isotopically labeled nucleic acids .
	manualset3
238886	5	421912	7	NULL	NULL	0	NULL	nitrogen resonances	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An efficient method is presented for the assignment of the proton , carbon , and nitrogen resonances in the NMR spectra of isotopically labeled nucleic acids .
	manualset3
238887	6	421912	7	NULL	NULL	0	NULL	NMR spectra	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An efficient method is presented for the assignment of the proton , carbon , and nitrogen resonances in the NMR spectra of isotopically labeled nucleic acids .
	manualset3
238888	7	421912	7	NULL	NULL	0	NULL	isotopically labeled nucleic acids	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	An efficient method is presented for the assignment of the proton , carbon , and nitrogen resonances in the NMR spectra of isotopically labeled nucleic acids .
	manualset3
238889	1	421913	7	NULL	NULL	0	NULL	Detection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Detection of simulated chest lesions with normal and reduced radiation dose : comparison of conventional screen-film radiography and a flat-panel x-ray detector based on amorphous silicon .
	manualset3
238890	2	421913	7	NULL	NULL	0	NULL	simulated chest lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Detection of simulated chest lesions with normal and reduced radiation dose : comparison of conventional screen-film radiography and a flat-panel x-ray detector based on amorphous silicon .
	manualset3
238891	3	421913	7	NULL	NULL	0	NULL	normal dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Detection of simulated chest lesions with normal and reduced radiation dose : comparison of conventional screen-film radiography and a flat-panel x-ray detector based on amorphous silicon .
	manualset3
238892	4	421913	7	NULL	NULL	0	NULL	reduced radiation dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Detection of simulated chest lesions with normal and reduced radiation dose : comparison of conventional screen-film radiography and a flat-panel x-ray detector based on amorphous silicon .
	manualset3
238893	5	421913	7	NULL	NULL	0	NULL	 comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Detection of simulated chest lesions with normal and reduced radiation dose : comparison of conventional screen-film radiography and a flat-panel x-ray detector based on amorphous silicon .
	manualset3
238894	6	421913	7	NULL	NULL	0	NULL	 conventional screen-film radiography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Detection of simulated chest lesions with normal and reduced radiation dose : comparison of conventional screen-film radiography and a flat-panel x-ray detector based on amorphous silicon .
	manualset3
238895	7	421913	7	NULL	NULL	0	NULL	flat-panel x-ray detector	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Detection of simulated chest lesions with normal and reduced radiation dose : comparison of conventional screen-film radiography and a flat-panel x-ray detector based on amorphous silicon .
	manualset3
238896	8	421913	7	NULL	NULL	0	NULL	amorphous silicon	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Detection of simulated chest lesions with normal and reduced radiation dose : comparison of conventional screen-film radiography and a flat-panel x-ray detector based on amorphous silicon .
	manualset3
238897	1	421914	7	NULL	NULL	0	NULL	molecular heterogeneity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular heterogeneity of both native AGP and desialylated AGP , based on Concanavalin A reactivity and isoelectric point , was not reflected by any specificity in the antibody reactions .
	manualset3
238898	2	421914	7	NULL	NULL	0	NULL	native AGP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular heterogeneity of both native AGP and desialylated AGP , based on Concanavalin A reactivity and isoelectric point , was not reflected by any specificity in the antibody reactions .
	manualset3
238899	3	421914	7	NULL	NULL	0	NULL	desialylated AGP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular heterogeneity of both native AGP and desialylated AGP , based on Concanavalin A reactivity and isoelectric point , was not reflected by any specificity in the antibody reactions .
	manualset3
238900	4	421914	7	NULL	NULL	0	NULL	Concanavalin A reactivity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular heterogeneity of both native AGP and desialylated AGP , based on Concanavalin A reactivity and isoelectric point , was not reflected by any specificity in the antibody reactions .
	manualset3
238901	5	421914	7	NULL	NULL	0	NULL	isoelectric point 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular heterogeneity of both native AGP and desialylated AGP , based on Concanavalin A reactivity and isoelectric point , was not reflected by any specificity in the antibody reactions .
	manualset3
238902	6	421914	7	NULL	NULL	0	NULL	antibody reactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The molecular heterogeneity of both native AGP and desialylated AGP , based on Concanavalin A reactivity and isoelectric point , was not reflected by any specificity in the antibody reactions .
	manualset3
238903	1	421915	7	NULL	NULL	0	NULL	Mutational analysis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutational analysis indicates that both predicted ATP binding domains in mdr1 are absolutely essential for biological activity .
	manualset3
238904	2	421915	7	NULL	NULL	0	NULL	predicted ATP binding domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutational analysis indicates that both predicted ATP binding domains in mdr1 are absolutely essential for biological activity .
	manualset3
238905	3	421915	7	NULL	NULL	0	NULL	mdr1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutational analysis indicates that both predicted ATP binding domains in mdr1 are absolutely essential for biological activity .
	manualset3
238906	4	421915	7	NULL	NULL	0	NULL	biological activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Mutational analysis indicates that both predicted ATP binding domains in mdr1 are absolutely essential for biological activity .
	manualset3
238907	1	421916	7	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine : 1 ) the effects of the HIV-1 envelope protein , gp-120 , on neonatal rat astrocytes in vitro ; 2 ) the spontaneous apoptosis of human neonatal and adult mononuclear leukocytes and , 3 ) the selective inhibition of NK activity cell from adult AIDS patients by the HIV-1 protein that caused brain pathology in neonatal rats .
	manualset3
238908	2	421916	7	NULL	NULL	0	NULL	HIV-1 envelope protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine : 1 ) the effects of the HIV-1 envelope protein , gp-120 , on neonatal rat astrocytes in vitro ; 2 ) the spontaneous apoptosis of human neonatal and adult mononuclear leukocytes and , 3 ) the selective inhibition of NK activity cell from adult AIDS patients by the HIV-1 protein that caused brain pathology in neonatal rats .
	manualset3
238909	3	421916	7	NULL	NULL	0	NULL	gp-120 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine : 1 ) the effects of the HIV-1 envelope protein , gp-120 , on neonatal rat astrocytes in vitro ; 2 ) the spontaneous apoptosis of human neonatal and adult mononuclear leukocytes and , 3 ) the selective inhibition of NK activity cell from adult AIDS patients by the HIV-1 protein that caused brain pathology in neonatal rats .
	manualset3
238910	4	421916	7	NULL	NULL	0	NULL	neonatal rat astrocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine : 1 ) the effects of the HIV-1 envelope protein , gp-120 , on neonatal rat astrocytes in vitro ; 2 ) the spontaneous apoptosis of human neonatal and adult mononuclear leukocytes and , 3 ) the selective inhibition of NK activity cell from adult AIDS patients by the HIV-1 protein that caused brain pathology in neonatal rats .
	manualset3
238911	5	421916	7	NULL	NULL	0	NULL	spontaneous apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine : 1 ) the effects of the HIV-1 envelope protein , gp-120 , on neonatal rat astrocytes in vitro ; 2 ) the spontaneous apoptosis of human neonatal and adult mononuclear leukocytes and , 3 ) the selective inhibition of NK activity cell from adult AIDS patients by the HIV-1 protein that caused brain pathology in neonatal rats .
	manualset3
238912	6	421916	7	NULL	NULL	0	NULL	 human neonatal leukocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine : 1 ) the effects of the HIV-1 envelope protein , gp-120 , on neonatal rat astrocytes in vitro ; 2 ) the spontaneous apoptosis of human neonatal and adult mononuclear leukocytes and , 3 ) the selective inhibition of NK activity cell from adult AIDS patients by the HIV-1 protein that caused brain pathology in neonatal rats .
	manualset3
238913	7	421916	7	NULL	NULL	0	NULL	adult mononuclear leukocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine : 1 ) the effects of the HIV-1 envelope protein , gp-120 , on neonatal rat astrocytes in vitro ; 2 ) the spontaneous apoptosis of human neonatal and adult mononuclear leukocytes and , 3 ) the selective inhibition of NK activity cell from adult AIDS patients by the HIV-1 protein that caused brain pathology in neonatal rats .
	manualset3
238914	8	421916	7	NULL	NULL	0	NULL	selective inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine : 1 ) the effects of the HIV-1 envelope protein , gp-120 , on neonatal rat astrocytes in vitro ; 2 ) the spontaneous apoptosis of human neonatal and adult mononuclear leukocytes and , 3 ) the selective inhibition of NK activity cell from adult AIDS patients by the HIV-1 protein that caused brain pathology in neonatal rats .
	manualset3
238915	9	421916	7	NULL	NULL	0	NULL	NK activity cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine : 1 ) the effects of the HIV-1 envelope protein , gp-120 , on neonatal rat astrocytes in vitro ; 2 ) the spontaneous apoptosis of human neonatal and adult mononuclear leukocytes and , 3 ) the selective inhibition of NK activity cell from adult AIDS patients by the HIV-1 protein that caused brain pathology in neonatal rats .
	manualset3
238916	10	421916	7	NULL	NULL	0	NULL	adult AIDS patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine : 1 ) the effects of the HIV-1 envelope protein , gp-120 , on neonatal rat astrocytes in vitro ; 2 ) the spontaneous apoptosis of human neonatal and adult mononuclear leukocytes and , 3 ) the selective inhibition of NK activity cell from adult AIDS patients by the HIV-1 protein that caused brain pathology in neonatal rats .
	manualset3
238917	11	421916	7	NULL	NULL	0	NULL	HIV-1 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine : 1 ) the effects of the HIV-1 envelope protein , gp-120 , on neonatal rat astrocytes in vitro ; 2 ) the spontaneous apoptosis of human neonatal and adult mononuclear leukocytes and , 3 ) the selective inhibition of NK activity cell from adult AIDS patients by the HIV-1 protein that caused brain pathology in neonatal rats .
	manualset3
238918	12	421916	7	NULL	NULL	0	NULL	brain pathology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine : 1 ) the effects of the HIV-1 envelope protein , gp-120 , on neonatal rat astrocytes in vitro ; 2 ) the spontaneous apoptosis of human neonatal and adult mononuclear leukocytes and , 3 ) the selective inhibition of NK activity cell from adult AIDS patients by the HIV-1 protein that caused brain pathology in neonatal rats .
	manualset3
238919	13	421916	7	NULL	NULL	0	NULL	neonatal rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we examine : 1 ) the effects of the HIV-1 envelope protein , gp-120 , on neonatal rat astrocytes in vitro ; 2 ) the spontaneous apoptosis of human neonatal and adult mononuclear leukocytes and , 3 ) the selective inhibition of NK activity cell from adult AIDS patients by the HIV-1 protein that caused brain pathology in neonatal rats .
	manualset3
238920	1	421917	7	NULL	NULL	0	NULL	HLA photoaffinity labeling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	HLA photoaffinity labeling reveals overlapping binding of homologous melanoma-associated gene peptides by HLA-A1 , HLA-A29 , and HLA-B44 .
	manualset3
238921	2	421917	7	NULL	NULL	0	NULL	overlapping binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HLA photoaffinity labeling reveals overlapping binding of homologous melanoma-associated gene peptides by HLA-A1 , HLA-A29 , and HLA-B44 .
	manualset3
238922	3	421917	7	NULL	NULL	NULL	NULL	homologous melanoma-associated gene peptides	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	HLA photoaffinity labeling reveals overlapping binding of homologous melanoma-associated gene peptides by HLA-A1 , HLA-A29 , and HLA-B44 .
	manualset3
238923	4	421917	7	NULL	NULL	0	NULL	homologous melanoma-associated gene peptides	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	HLA photoaffinity labeling reveals overlapping binding of homologous melanoma-associated gene peptides by HLA-A1 , HLA-A29 , and HLA-B44 .
	manualset3
238924	5	421917	7	NULL	NULL	0	NULL	HLA-A1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	HLA photoaffinity labeling reveals overlapping binding of homologous melanoma-associated gene peptides by HLA-A1 , HLA-A29 , and HLA-B44 .
	manualset3
238925	6	421917	7	NULL	NULL	0	NULL	HLA-A29	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	HLA photoaffinity labeling reveals overlapping binding of homologous melanoma-associated gene peptides by HLA-A1 , HLA-A29 , and HLA-B44 .
	manualset3
238926	7	421917	7	NULL	NULL	0	NULL	HLA-B44	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	HLA photoaffinity labeling reveals overlapping binding of homologous melanoma-associated gene peptides by HLA-A1 , HLA-A29 , and HLA-B44 .
	manualset3
238927	1	421918	7	NULL	NULL	0	NULL	STAT5 Protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	STAT5 Protein Negatively Regulates T Follicular Helper ( Tfh ) Cell Generation and Function .
	manualset3
238928	2	421918	7	NULL	NULL	0	NULL	T Follicular Helper ( Tfh ) Cell Generation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	STAT5 Protein Negatively Regulates T Follicular Helper ( Tfh ) Cell Generation and Function .
	manualset3
238929	3	421918	7	NULL	NULL	0	NULL	Function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	STAT5 Protein Negatively Regulates T Follicular Helper ( Tfh ) Cell Generation and Function .
	manualset3
238930	1	421919	7	NULL	NULL	0	NULL	Intensive treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intensive treatment of patients age 60 years and older with de novo acute myeloid leukemia : analysis of prognostic factors .
	manualset3
238931	2	421919	7	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Intensive treatment of patients age 60 years and older with de novo acute myeloid leukemia : analysis of prognostic factors .
	manualset3
238932	3	421919	7	NULL	NULL	0	NULL	age 60 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Intensive treatment of patients age 60 years and older with de novo acute myeloid leukemia : analysis of prognostic factors .
	manualset3
238933	4	421919	7	NULL	NULL	0	NULL	de novo acute myeloid leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Intensive treatment of patients age 60 years and older with de novo acute myeloid leukemia : analysis of prognostic factors .
	manualset3
238934	5	421919	7	NULL	NULL	0	NULL	analysis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Intensive treatment of patients age 60 years and older with de novo acute myeloid leukemia : analysis of prognostic factors .
	manualset3
238935	6	421919	7	NULL	NULL	0	NULL	prognostic factors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Intensive treatment of patients age 60 years and older with de novo acute myeloid leukemia : analysis of prognostic factors .
	manualset3
238936	1	421920	7	NULL	NULL	0	NULL	Progesterone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Progesterone represses interleukin-8 and cyclo-oxygenase-2 in human lower segment fibroblast cells and amnion epithelial cells .
	manualset3
238937	2	421920	7	NULL	NULL	0	NULL	interleukin-8	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Progesterone represses interleukin-8 and cyclo-oxygenase-2 in human lower segment fibroblast cells and amnion epithelial cells .
	manualset3
238938	3	421920	7	NULL	NULL	0	NULL	cyclo-oxygenase-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Progesterone represses interleukin-8 and cyclo-oxygenase-2 in human lower segment fibroblast cells and amnion epithelial cells .
	manualset3
238939	4	421920	7	NULL	NULL	0	NULL	human lower segment fibroblast cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Progesterone represses interleukin-8 and cyclo-oxygenase-2 in human lower segment fibroblast cells and amnion epithelial cells .
	manualset3
238940	5	421920	7	NULL	NULL	0	NULL	amnion epithelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Progesterone represses interleukin-8 and cyclo-oxygenase-2 in human lower segment fibroblast cells and amnion epithelial cells .
	manualset3
238941	1	421921	7	NULL	NULL	0	NULL	Infrared study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Infrared study of the CH stretching bands of chlorophyll a and of chlorophyll b in monolayers .
	manualset3
238942	2	421921	7	NULL	NULL	0	NULL	CH stretching bands	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Infrared study of the CH stretching bands of chlorophyll a and of chlorophyll b in monolayers .
	manualset3
238943	3	421921	7	NULL	NULL	0	NULL	chlorophyll a 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Infrared study of the CH stretching bands of chlorophyll a and of chlorophyll b in monolayers .
	manualset3
238944	4	421921	7	NULL	NULL	0	NULL	chlorophyll b	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Infrared study of the CH stretching bands of chlorophyll a and of chlorophyll b in monolayers .
	manualset3
238945	5	421921	7	NULL	NULL	0	NULL	monolayers	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Infrared study of the CH stretching bands of chlorophyll a and of chlorophyll b in monolayers .
	manualset3
238949	1	421922	7	NULL	NULL	0	NULL	role 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of free hydroxyproline in the biosynthesis of collagen .
	manualset3
238951	2	421922	7	NULL	NULL	0	NULL	free hydroxyproline	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of free hydroxyproline in the biosynthesis of collagen .
	manualset3
238953	3	421922	7	NULL	NULL	0	NULL	biosynthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of free hydroxyproline in the biosynthesis of collagen .
	manualset3
238955	4	421922	7	NULL	NULL	0	NULL	collagen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The role of free hydroxyproline in the biosynthesis of collagen .
	manualset3
238957	1	421923	7	NULL	NULL	0	NULL	DA systems	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , while DA systems appear to be a critical link , not only in the acute effects of AMPH , but also in the development of tolerance and reverse tolerance , most of the behavioral differences between acutely and chronically treated animals are not reflected by comparable differences in DA synthesis and metabolism .
	manualset3
238958	2	421923	7	NULL	NULL	0	NULL	acute effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , while DA systems appear to be a critical link , not only in the acute effects of AMPH , but also in the development of tolerance and reverse tolerance , most of the behavioral differences between acutely and chronically treated animals are not reflected by comparable differences in DA synthesis and metabolism .
	manualset3
238959	3	421923	7	NULL	NULL	0	NULL	AMPH	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , while DA systems appear to be a critical link , not only in the acute effects of AMPH , but also in the development of tolerance and reverse tolerance , most of the behavioral differences between acutely and chronically treated animals are not reflected by comparable differences in DA synthesis and metabolism .
	manualset3
238960	4	421923	7	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , while DA systems appear to be a critical link , not only in the acute effects of AMPH , but also in the development of tolerance and reverse tolerance , most of the behavioral differences between acutely and chronically treated animals are not reflected by comparable differences in DA synthesis and metabolism .
	manualset3
238961	5	421923	7	NULL	NULL	0	NULL	behavioral differences	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , while DA systems appear to be a critical link , not only in the acute effects of AMPH , but also in the development of tolerance and reverse tolerance , most of the behavioral differences between acutely and chronically treated animals are not reflected by comparable differences in DA synthesis and metabolism .
	manualset3
238962	6	421923	7	NULL	NULL	0	NULL	chronically treated animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , while DA systems appear to be a critical link , not only in the acute effects of AMPH , but also in the development of tolerance and reverse tolerance , most of the behavioral differences between acutely and chronically treated animals are not reflected by comparable differences in DA synthesis and metabolism .
	manualset3
238963	7	421923	7	NULL	NULL	0	NULL	comparable differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , while DA systems appear to be a critical link , not only in the acute effects of AMPH , but also in the development of tolerance and reverse tolerance , most of the behavioral differences between acutely and chronically treated animals are not reflected by comparable differences in DA synthesis and metabolism .
	manualset3
238964	8	421923	7	NULL	NULL	0	NULL	DA synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , while DA systems appear to be a critical link , not only in the acute effects of AMPH , but also in the development of tolerance and reverse tolerance , most of the behavioral differences between acutely and chronically treated animals are not reflected by comparable differences in DA synthesis and metabolism .
	manualset3
238965	9	421923	7	NULL	NULL	0	NULL	metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , while DA systems appear to be a critical link , not only in the acute effects of AMPH , but also in the development of tolerance and reverse tolerance , most of the behavioral differences between acutely and chronically treated animals are not reflected by comparable differences in DA synthesis and metabolism .
	manualset3
238970	1	421924	7	NULL	NULL	0	NULL	magnesium-orotate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Does magnesium-orotate improve the effect of lipid lowering drugs ? ) .
	manualset3
238971	2	421924	7	NULL	NULL	0	NULL	 effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Does magnesium-orotate improve the effect of lipid lowering drugs ? ) .
	manualset3
238972	3	421924	7	NULL	NULL	0	NULL	lipid lowering drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Does magnesium-orotate improve the effect of lipid lowering drugs ? ) .
	manualset3
238973	1	421925	7	NULL	NULL	0	NULL	Epidemiological studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiological studies have established a strong association between obstetric exposure to diagnostic radiation and an increase in the incidence of childhood leukemia and between low dose gamma irradiation during the early fetal period and mental retardation in children .
	manualset3
238974	2	421925	7	NULL	NULL	0	NULL	strong association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiological studies have established a strong association between obstetric exposure to diagnostic radiation and an increase in the incidence of childhood leukemia and between low dose gamma irradiation during the early fetal period and mental retardation in children .
	manualset3
238975	3	421925	7	NULL	NULL	0	NULL	obstetric exposure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiological studies have established a strong association between obstetric exposure to diagnostic radiation and an increase in the incidence of childhood leukemia and between low dose gamma irradiation during the early fetal period and mental retardation in children .
	manualset3
238976	4	421925	7	NULL	NULL	NULL	NULL	diagnostic radiation 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Epidemiological studies have established a strong association between obstetric exposure to diagnostic radiation and an increase in the incidence of childhood leukemia and between low dose gamma irradiation during the early fetal period and mental retardation in children .
	manualset3
238977	5	421925	7	NULL	NULL	0	NULL	incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiological studies have established a strong association between obstetric exposure to diagnostic radiation and an increase in the incidence of childhood leukemia and between low dose gamma irradiation during the early fetal period and mental retardation in children .
	manualset3
238979	6	421925	7	NULL	NULL	0	NULL	childhood leukemia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiological studies have established a strong association between obstetric exposure to diagnostic radiation and an increase in the incidence of childhood leukemia and between low dose gamma irradiation during the early fetal period and mental retardation in children .
	manualset3
238980	7	421925	7	NULL	NULL	NULL	NULL	low dose gamma irradiation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Epidemiological studies have established a strong association between obstetric exposure to diagnostic radiation and an increase in the incidence of childhood leukemia and between low dose gamma irradiation during the early fetal period and mental retardation in children .
	manualset3
238981	8	421925	7	NULL	NULL	0	NULL	early fetal period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiological studies have established a strong association between obstetric exposure to diagnostic radiation and an increase in the incidence of childhood leukemia and between low dose gamma irradiation during the early fetal period and mental retardation in children .
	manualset3
238982	9	421925	7	NULL	NULL	0	NULL	mental retardation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiological studies have established a strong association between obstetric exposure to diagnostic radiation and an increase in the incidence of childhood leukemia and between low dose gamma irradiation during the early fetal period and mental retardation in children .
	manualset3
238983	10	421925	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiological studies have established a strong association between obstetric exposure to diagnostic radiation and an increase in the incidence of childhood leukemia and between low dose gamma irradiation during the early fetal period and mental retardation in children .
	manualset3
242899	11	421925	7	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Epidemiological studies have established a strong association between obstetric exposure to diagnostic radiation and an increase in the incidence of childhood leukemia and between low dose gamma irradiation during the early fetal period and mental retardation in children .
	manualset3
238984	1	421926	7	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of an increase in Ca + + from the control level of 1.5 mmol/liter to 2.25 , 3.0 , and 4.5 mmol/liter was tested in random order in five thyroid lobes .
	manualset3
238985	2	421926	7	NULL	NULL	0	NULL	 increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of an increase in Ca + + from the control level of 1.5 mmol/liter to 2.25 , 3.0 , and 4.5 mmol/liter was tested in random order in five thyroid lobes .
	manualset3
238986	3	421926	7	NULL	NULL	0	NULL	Ca + + 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of an increase in Ca + + from the control level of 1.5 mmol/liter to 2.25 , 3.0 , and 4.5 mmol/liter was tested in random order in five thyroid lobes .
	manualset3
238987	4	421926	7	NULL	NULL	0	NULL	control level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of an increase in Ca + + from the control level of 1.5 mmol/liter to 2.25 , 3.0 , and 4.5 mmol/liter was tested in random order in five thyroid lobes .
	manualset3
238988	5	421926	7	NULL	NULL	0	NULL	1.5 mmol/liter 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of an increase in Ca + + from the control level of 1.5 mmol/liter to 2.25 , 3.0 , and 4.5 mmol/liter was tested in random order in five thyroid lobes .
	manualset3
238989	6	421926	7	NULL	NULL	0	NULL	2.25 mmol/liter	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of an increase in Ca + + from the control level of 1.5 mmol/liter to 2.25 , 3.0 , and 4.5 mmol/liter was tested in random order in five thyroid lobes .
	manualset3
238990	7	421926	7	NULL	NULL	0	NULL	3.0 mmol/liter	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of an increase in Ca + + from the control level of 1.5 mmol/liter to 2.25 , 3.0 , and 4.5 mmol/liter was tested in random order in five thyroid lobes .
	manualset3
238991	8	421926	7	NULL	NULL	0	NULL	4.5 mmol/liter	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of an increase in Ca + + from the control level of 1.5 mmol/liter to 2.25 , 3.0 , and 4.5 mmol/liter was tested in random order in five thyroid lobes .
	manualset3
238992	9	421926	7	NULL	NULL	0	NULL	random order	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of an increase in Ca + + from the control level of 1.5 mmol/liter to 2.25 , 3.0 , and 4.5 mmol/liter was tested in random order in five thyroid lobes .
	manualset3
238993	10	421926	7	NULL	NULL	0	NULL	five thyroid lobes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of an increase in Ca + + from the control level of 1.5 mmol/liter to 2.25 , 3.0 , and 4.5 mmol/liter was tested in random order in five thyroid lobes .
	manualset3
238994	1	421927	7	NULL	NULL	0	NULL	 sulfurylase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Both sulfurylase and kinase from rat chondrosarcoma were copurified through substrate affinity chromatography using stable analogs of APS ( adenosine 5 ' - phosphosulfate ) and PAPS ( 3 ' - phosphoadenosine 5 ' - phosphosulfate ) .
	manualset3
238995	2	421927	7	NULL	NULL	0	NULL	kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Both sulfurylase and kinase from rat chondrosarcoma were copurified through substrate affinity chromatography using stable analogs of APS ( adenosine 5 ' - phosphosulfate ) and PAPS ( 3 ' - phosphoadenosine 5 ' - phosphosulfate ) .
	manualset3
238996	3	421927	7	NULL	NULL	0	NULL	rat chondrosarcoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Both sulfurylase and kinase from rat chondrosarcoma were copurified through substrate affinity chromatography using stable analogs of APS ( adenosine 5 ' - phosphosulfate ) and PAPS ( 3 ' - phosphoadenosine 5 ' - phosphosulfate ) .
	manualset3
238997	4	421927	7	NULL	NULL	0	NULL	substrate affinity chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Both sulfurylase and kinase from rat chondrosarcoma were copurified through substrate affinity chromatography using stable analogs of APS ( adenosine 5 ' - phosphosulfate ) and PAPS ( 3 ' - phosphoadenosine 5 ' - phosphosulfate ) .
	manualset3
238998	5	421927	7	NULL	NULL	0	NULL	 stable analogs 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Both sulfurylase and kinase from rat chondrosarcoma were copurified through substrate affinity chromatography using stable analogs of APS ( adenosine 5 ' - phosphosulfate ) and PAPS ( 3 ' - phosphoadenosine 5 ' - phosphosulfate ) .
	manualset3
238999	6	421927	7	NULL	NULL	0	NULL	APS ( adenosine 5 ' - phosphosulfate )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Both sulfurylase and kinase from rat chondrosarcoma were copurified through substrate affinity chromatography using stable analogs of APS ( adenosine 5 ' - phosphosulfate ) and PAPS ( 3 ' - phosphoadenosine 5 ' - phosphosulfate ) .
	manualset3
239000	7	421927	7	NULL	NULL	0	NULL	PAPS ( 3 ' - phosphoadenosine 5 ' - phosphosulfate )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Both sulfurylase and kinase from rat chondrosarcoma were copurified through substrate affinity chromatography using stable analogs of APS ( adenosine 5 ' - phosphosulfate ) and PAPS ( 3 ' - phosphoadenosine 5 ' - phosphosulfate ) .
	manualset3
239001	1	421928	7	NULL	NULL	0	NULL	Arachidonate	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Arachidonate stimulated NADPH oxidase activity accompanied by a marked phosphorylation of membrane proteins .
	manualset3
239002	2	421928	7	NULL	NULL	0	NULL	NADPH oxidase activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Arachidonate stimulated NADPH oxidase activity accompanied by a marked phosphorylation of membrane proteins .
	manualset3
239003	3	421928	7	NULL	NULL	0	NULL	marked phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Arachidonate stimulated NADPH oxidase activity accompanied by a marked phosphorylation of membrane proteins .
	manualset3
239004	4	421928	7	NULL	NULL	0	NULL	membrane proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Arachidonate stimulated NADPH oxidase activity accompanied by a marked phosphorylation of membrane proteins .
	manualset3
239005	1	421929	7	NULL	NULL	0	NULL	Respiratory muscle activity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Respiratory muscle activity in patients with COPD walking to exhaustion with and without pressure support .
	manualset3
239006	2	421929	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Respiratory muscle activity in patients with COPD walking to exhaustion with and without pressure support .
	manualset3
239007	3	421929	7	NULL	NULL	0	NULL	COPD walking	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Respiratory muscle activity in patients with COPD walking to exhaustion with and without pressure support .
	manualset3
239008	4	421929	7	NULL	NULL	0	NULL	exhaustion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Respiratory muscle activity in patients with COPD walking to exhaustion with and without pressure support .
	manualset3
239009	5	421929	7	NULL	NULL	0	NULL	pressure support 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Respiratory muscle activity in patients with COPD walking to exhaustion with and without pressure support .
	manualset3
239010	1	421930	7	NULL	NULL	0	NULL	 valproate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrate that , in the presence of valproate , glutamate consumption and aspartate accumulation and labeling were inhibited , whereas GABA accumulation and labeling were increased .
	manualset3
239011	2	421930	7	NULL	NULL	0	NULL	glutamate consumption 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrate that , in the presence of valproate , glutamate consumption and aspartate accumulation and labeling were inhibited , whereas GABA accumulation and labeling were increased .
	manualset3
239012	3	421930	7	NULL	NULL	NULL	NULL	aspartate accumulation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We demonstrate that , in the presence of valproate , glutamate consumption and aspartate accumulation and labeling were inhibited , whereas GABA accumulation and labeling were increased .
	manualset3
239013	4	421930	7	NULL	NULL	0	NULL	labeling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrate that , in the presence of valproate , glutamate consumption and aspartate accumulation and labeling were inhibited , whereas GABA accumulation and labeling were increased .
	manualset3
239015	5	421930	7	NULL	NULL	0	NULL	GABA accumulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrate that , in the presence of valproate , glutamate consumption and aspartate accumulation and labeling were inhibited , whereas GABA accumulation and labeling were increased .
	manualset3
239016	6	421930	7	NULL	NULL	0	NULL	labeling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We demonstrate that , in the presence of valproate , glutamate consumption and aspartate accumulation and labeling were inhibited , whereas GABA accumulation and labeling were increased .
	manualset3
239590	1	421931	7	NULL	NULL	0	NULL	resonance energy transfer ( RET ) assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We applied resonance energy transfer ( RET ) assays to analyze the fusogenic properties of this peptide by lipid mixing and used liposomes containing carboxyfluorescein to measure the contents leakage .
	manualset3
239591	2	421931	7	NULL	NULL	0	NULL	fusogenic properties	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We applied resonance energy transfer ( RET ) assays to analyze the fusogenic properties of this peptide by lipid mixing and used liposomes containing carboxyfluorescein to measure the contents leakage .
	manualset3
239592	3	421931	7	NULL	NULL	0	NULL	 peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	We applied resonance energy transfer ( RET ) assays to analyze the fusogenic properties of this peptide by lipid mixing and used liposomes containing carboxyfluorescein to measure the contents leakage .
	manualset3
239593	4	421931	7	NULL	NULL	0	NULL	lipid mixing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We applied resonance energy transfer ( RET ) assays to analyze the fusogenic properties of this peptide by lipid mixing and used liposomes containing carboxyfluorescein to measure the contents leakage .
	manualset3
239594	5	421931	7	NULL	NULL	NULL	NULL	liposomes	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We applied resonance energy transfer ( RET ) assays to analyze the fusogenic properties of this peptide by lipid mixing and used liposomes containing carboxyfluorescein to measure the contents leakage .
	manualset3
239595	6	421931	7	NULL	NULL	0	NULL	carboxyfluorescein	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We applied resonance energy transfer ( RET ) assays to analyze the fusogenic properties of this peptide by lipid mixing and used liposomes containing carboxyfluorescein to measure the contents leakage .
	manualset3
239596	7	421931	7	NULL	NULL	0	NULL	contents leakage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We applied resonance energy transfer ( RET ) assays to analyze the fusogenic properties of this peptide by lipid mixing and used liposomes containing carboxyfluorescein to measure the contents leakage .
	manualset3
239597	1	421932	7	NULL	NULL	0	NULL	Response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Response of two strains of rats to a high-protein diet containing sucrose or cornstarch .
	manualset3
239598	2	421932	7	NULL	NULL	0	NULL	two strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Response of two strains of rats to a high-protein diet containing sucrose or cornstarch .
	manualset3
239599	3	421932	7	NULL	NULL	0	NULL	 rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Response of two strains of rats to a high-protein diet containing sucrose or cornstarch .
	manualset3
239600	4	421932	7	NULL	NULL	0	NULL	high-protein diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Response of two strains of rats to a high-protein diet containing sucrose or cornstarch .
	manualset3
239601	5	421932	7	NULL	NULL	0	NULL	sucrose	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Response of two strains of rats to a high-protein diet containing sucrose or cornstarch .
	manualset3
239602	6	421932	7	NULL	NULL	0	NULL	cornstarch 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Response of two strains of rats to a high-protein diet containing sucrose or cornstarch .
	manualset3
239657	1	421933	7	NULL	NULL	0	NULL	Induction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of vascular remodeling in the lung by chronic house dust mite exposure .
	manualset3
239658	2	421933	7	NULL	NULL	0	NULL	vascular remodeling	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of vascular remodeling in the lung by chronic house dust mite exposure .
	manualset3
239659	3	421933	7	NULL	NULL	0	NULL	 lung	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of vascular remodeling in the lung by chronic house dust mite exposure .
	manualset3
239660	4	421933	7	NULL	NULL	0	NULL	chronic house dust mite exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Induction of vascular remodeling in the lung by chronic house dust mite exposure .
	manualset3
239661	1	421934	7	NULL	NULL	0	NULL	Water structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Water structure was perturbed by a series of reagents known to affect the phase equilibrium of lipid assemblies .
	manualset3
239662	2	421934	7	NULL	NULL	0	NULL	series	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Water structure was perturbed by a series of reagents known to affect the phase equilibrium of lipid assemblies .
	manualset3
239663	3	421934	7	NULL	NULL	0	NULL	reagents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Water structure was perturbed by a series of reagents known to affect the phase equilibrium of lipid assemblies .
	manualset3
239664	4	421934	7	NULL	NULL	0	NULL	 phase equilibrium	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Water structure was perturbed by a series of reagents known to affect the phase equilibrium of lipid assemblies .
	manualset3
239665	5	421934	7	NULL	NULL	0	NULL	lipid assemblies	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Water structure was perturbed by a series of reagents known to affect the phase equilibrium of lipid assemblies .
	manualset3
239674	1	421935	7	NULL	NULL	0	NULL	alphaxolone 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The alphaxolone showed a DRSM very low ( 0.489 ) on the contrary the dose of thiopentone required to obtain no sympathetic response is high ( 7.776 ) .
	manualset3
239675	2	421935	7	NULL	NULL	0	NULL	DRSM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The alphaxolone showed a DRSM very low ( 0.489 ) on the contrary the dose of thiopentone required to obtain no sympathetic response is high ( 7.776 ) .
	manualset3
239676	3	421935	7	NULL	NULL	0	NULL	 0.489	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The alphaxolone showed a DRSM very low ( 0.489 ) on the contrary the dose of thiopentone required to obtain no sympathetic response is high ( 7.776 ) .
	manualset3
239677	4	421935	7	NULL	NULL	0	NULL	 dose 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The alphaxolone showed a DRSM very low ( 0.489 ) on the contrary the dose of thiopentone required to obtain no sympathetic response is high ( 7.776 ) .
	manualset3
239678	5	421935	7	NULL	NULL	0	NULL	thiopentone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The alphaxolone showed a DRSM very low ( 0.489 ) on the contrary the dose of thiopentone required to obtain no sympathetic response is high ( 7.776 ) .
	manualset3
239679	6	421935	7	NULL	NULL	0	NULL	no sympathetic response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The alphaxolone showed a DRSM very low ( 0.489 ) on the contrary the dose of thiopentone required to obtain no sympathetic response is high ( 7.776 ) .
	manualset3
239680	7	421935	7	NULL	NULL	0	NULL	7.776	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The alphaxolone showed a DRSM very low ( 0.489 ) on the contrary the dose of thiopentone required to obtain no sympathetic response is high ( 7.776 ) .
	manualset3
239681	1	421936	7	NULL	NULL	0	NULL	 increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further increase in amount or intensity of physical activity above the minimal recommendations improves the morbidity preventive effect further , although several risk factors show a curvelinear and levelling-off pattern of their dosis-response curve between training and risk factors .
	manualset3
239682	2	421936	7	NULL	NULL	0	NULL	intensity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Further increase in amount or intensity of physical activity above the minimal recommendations improves the morbidity preventive effect further , although several risk factors show a curvelinear and levelling-off pattern of their dosis-response curve between training and risk factors .
	manualset3
239683	3	421936	7	NULL	NULL	0	NULL	physical activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Further increase in amount or intensity of physical activity above the minimal recommendations improves the morbidity preventive effect further , although several risk factors show a curvelinear and levelling-off pattern of their dosis-response curve between training and risk factors .
	manualset3
239684	4	421936	7	NULL	NULL	0	NULL	minimal recommendations 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further increase in amount or intensity of physical activity above the minimal recommendations improves the morbidity preventive effect further , although several risk factors show a curvelinear and levelling-off pattern of their dosis-response curve between training and risk factors .
	manualset3
239685	5	421936	7	NULL	NULL	0	NULL	morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Further increase in amount or intensity of physical activity above the minimal recommendations improves the morbidity preventive effect further , although several risk factors show a curvelinear and levelling-off pattern of their dosis-response curve between training and risk factors .
	manualset3
239686	6	421936	7	NULL	NULL	0	NULL	risk factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Further increase in amount or intensity of physical activity above the minimal recommendations improves the morbidity preventive effect further , although several risk factors show a curvelinear and levelling-off pattern of their dosis-response curve between training and risk factors .
	manualset3
239687	7	421936	7	NULL	NULL	0	NULL	curvelinear pattern	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further increase in amount or intensity of physical activity above the minimal recommendations improves the morbidity preventive effect further , although several risk factors show a curvelinear and levelling-off pattern of their dosis-response curve between training and risk factors .
	manualset3
239688	8	421936	7	NULL	NULL	0	NULL	levelling-off pattern 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further increase in amount or intensity of physical activity above the minimal recommendations improves the morbidity preventive effect further , although several risk factors show a curvelinear and levelling-off pattern of their dosis-response curve between training and risk factors .
	manualset3
239689	9	421936	7	NULL	NULL	0	NULL	dosis-response curve	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Further increase in amount or intensity of physical activity above the minimal recommendations improves the morbidity preventive effect further , although several risk factors show a curvelinear and levelling-off pattern of their dosis-response curve between training and risk factors .
	manualset3
239690	10	421936	7	NULL	NULL	0	NULL	training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further increase in amount or intensity of physical activity above the minimal recommendations improves the morbidity preventive effect further , although several risk factors show a curvelinear and levelling-off pattern of their dosis-response curve between training and risk factors .
	manualset3
239691	11	421936	7	NULL	NULL	0	NULL	risk factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Further increase in amount or intensity of physical activity above the minimal recommendations improves the morbidity preventive effect further , although several risk factors show a curvelinear and levelling-off pattern of their dosis-response curve between training and risk factors .
	manualset3
239692	12	421936	7	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Further increase in amount or intensity of physical activity above the minimal recommendations improves the morbidity preventive effect further , although several risk factors show a curvelinear and levelling-off pattern of their dosis-response curve between training and risk factors .
	manualset3
239693	1	421937	7	NULL	NULL	0	NULL	 determination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the determination of CMV-IgG-specific antibodies seems to be sufficient for routine CMV screening in blood donor centers .
	manualset3
239694	2	421937	7	NULL	NULL	0	NULL	CMV-IgG-specific antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the determination of CMV-IgG-specific antibodies seems to be sufficient for routine CMV screening in blood donor centers .
	manualset3
239695	3	421937	7	NULL	NULL	0	NULL	routine CMV screening	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the determination of CMV-IgG-specific antibodies seems to be sufficient for routine CMV screening in blood donor centers .
	manualset3
239696	4	421937	7	NULL	NULL	0	NULL	blood donor centers	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the determination of CMV-IgG-specific antibodies seems to be sufficient for routine CMV screening in blood donor centers .
	manualset3
239697	1	421938	7	NULL	NULL	0	NULL	Two complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two complications related to the ketogenic diet are selenium deficiency , which has been associated with impaired myocardial function , and QT prolongation as documented on electrocardiography .
	manualset3
239698	2	421938	7	NULL	NULL	0	NULL	ketogenic diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Two complications related to the ketogenic diet are selenium deficiency , which has been associated with impaired myocardial function , and QT prolongation as documented on electrocardiography .
	manualset3
239699	3	421938	7	NULL	NULL	0	NULL	selenium deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two complications related to the ketogenic diet are selenium deficiency , which has been associated with impaired myocardial function , and QT prolongation as documented on electrocardiography .
	manualset3
239700	4	421938	7	NULL	NULL	0	NULL	impaired myocardial function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two complications related to the ketogenic diet are selenium deficiency , which has been associated with impaired myocardial function , and QT prolongation as documented on electrocardiography .
	manualset3
239701	5	421938	7	NULL	NULL	0	NULL	QT prolongation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two complications related to the ketogenic diet are selenium deficiency , which has been associated with impaired myocardial function , and QT prolongation as documented on electrocardiography .
	manualset3
239702	6	421938	7	NULL	NULL	0	NULL	electrocardiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Two complications related to the ketogenic diet are selenium deficiency , which has been associated with impaired myocardial function , and QT prolongation as documented on electrocardiography .
	manualset3
240150	1	421939	7	NULL	NULL	0	NULL	electrocatalytic glucose sensor	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	An electrocatalytic glucose sensor for in vivo application has been developed to determine the glucose level in blood and further to control the insulin dosage in a closed loop system for diabetes therapy .
	manualset3
240151	2	421939	7	NULL	NULL	0	NULL	in vivo application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An electrocatalytic glucose sensor for in vivo application has been developed to determine the glucose level in blood and further to control the insulin dosage in a closed loop system for diabetes therapy .
	manualset3
240152	3	421939	7	NULL	NULL	0	NULL	glucose level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An electrocatalytic glucose sensor for in vivo application has been developed to determine the glucose level in blood and further to control the insulin dosage in a closed loop system for diabetes therapy .
	manualset3
240153	4	421939	7	NULL	NULL	0	NULL	blood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An electrocatalytic glucose sensor for in vivo application has been developed to determine the glucose level in blood and further to control the insulin dosage in a closed loop system for diabetes therapy .
	manualset3
240154	5	421939	7	NULL	NULL	0	NULL	insulin dosage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An electrocatalytic glucose sensor for in vivo application has been developed to determine the glucose level in blood and further to control the insulin dosage in a closed loop system for diabetes therapy .
	manualset3
240155	6	421939	7	NULL	NULL	0	NULL	closed loop system	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An electrocatalytic glucose sensor for in vivo application has been developed to determine the glucose level in blood and further to control the insulin dosage in a closed loop system for diabetes therapy .
	manualset3
240156	7	421939	7	NULL	NULL	0	NULL	diabetes therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An electrocatalytic glucose sensor for in vivo application has been developed to determine the glucose level in blood and further to control the insulin dosage in a closed loop system for diabetes therapy .
	manualset3
240157	1	421940	7	NULL	NULL	NULL	NULL	Particles	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Particles indistinguishable from the previously elusive provirions were observed ; these particles have been proposed to be penultimate in virion morphogenesis .
	manualset3
240158	2	421940	7	NULL	NULL	0	NULL	 provirions	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Particles indistinguishable from the previously elusive provirions were observed ; these particles have been proposed to be penultimate in virion morphogenesis .
	manualset3
240159	3	421940	7	NULL	NULL	0	NULL	 particles	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Particles indistinguishable from the previously elusive provirions were observed ; these particles have been proposed to be penultimate in virion morphogenesis .
	manualset3
240160	4	421940	7	NULL	NULL	0	NULL	virion morphogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Particles indistinguishable from the previously elusive provirions were observed ; these particles have been proposed to be penultimate in virion morphogenesis .
	manualset3
240161	1	421941	7	NULL	NULL	0	NULL	Thermal stability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermal stability of organic adsorbents used for sintered thin-layer chromatography ( author 's transl ) ) .
	manualset3
240162	2	421941	7	NULL	NULL	0	NULL	organic adsorbents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermal stability of organic adsorbents used for sintered thin-layer chromatography ( author 's transl ) ) .
	manualset3
240163	3	421941	7	NULL	NULL	0	NULL	 sintered thin-layer chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermal stability of organic adsorbents used for sintered thin-layer chromatography ( author 's transl ) ) .
	manualset3
240164	4	421941	7	NULL	NULL	0	NULL	author 's transl	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	Thermal stability of organic adsorbents used for sintered thin-layer chromatography ( author 's transl ) ) .
	manualset3
240165	1	421942	7	NULL	NULL	0	NULL	Correction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Correction of a severely rotated maxillary central incisor with the Whip device .
	manualset3
240166	2	421942	7	NULL	NULL	0	NULL	severely rotated maxillary central incisor	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Correction of a severely rotated maxillary central incisor with the Whip device .
	manualset3
240167	3	421942	7	NULL	NULL	0	NULL	Whip device	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Correction of a severely rotated maxillary central incisor with the Whip device .
	manualset3
240168	1	421943	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Based on the results obtained , we determined whether or not the given fragment is a processing site .
	manualset3
240169	2	421943	7	NULL	NULL	NULL	NULL	given fragment	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the results obtained , we determined whether or not the given fragment is a processing site .
	manualset3
240170	3	421943	7	NULL	NULL	NULL	NULL	processing site	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the results obtained , we determined whether or not the given fragment is a processing site .
	manualset3
240171	1	421944	7	NULL	NULL	0	NULL	sheath cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The sheath cells and their processes which first delineate axon bundles from one another form a network in the interstices of which lie the emergent axon bundles .
	manualset3
240172	2	421944	7	NULL	NULL	0	NULL	processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The sheath cells and their processes which first delineate axon bundles from one another form a network in the interstices of which lie the emergent axon bundles .
	manualset3
240173	3	421944	7	NULL	NULL	0	NULL	axon bundles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The sheath cells and their processes which first delineate axon bundles from one another form a network in the interstices of which lie the emergent axon bundles .
	manualset3
240174	4	421944	7	NULL	NULL	0	NULL	network	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The sheath cells and their processes which first delineate axon bundles from one another form a network in the interstices of which lie the emergent axon bundles .
	manualset3
240175	5	421944	7	NULL	NULL	0	NULL	interstices	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The sheath cells and their processes which first delineate axon bundles from one another form a network in the interstices of which lie the emergent axon bundles .
	manualset3
240176	6	421944	7	NULL	NULL	0	NULL	emergent axon bundles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The sheath cells and their processes which first delineate axon bundles from one another form a network in the interstices of which lie the emergent axon bundles .
	manualset3
240177	7	421944	7	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The sheath cells and their processes which first delineate axon bundles from one another form a network in the interstices of which lie the emergent axon bundles .
	manualset3
240178	1	421945	7	NULL	NULL	0	NULL	cellulase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The cellulase from steam-pretreated Lespedeza was found to have the most efficient hydrolysis capability to this specific substrate .
	manualset3
240179	2	421945	7	NULL	NULL	0	NULL	steam-pretreated Lespedeza	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The cellulase from steam-pretreated Lespedeza was found to have the most efficient hydrolysis capability to this specific substrate .
	manualset3
240180	3	421945	7	NULL	NULL	0	NULL	efficient hydrolysis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cellulase from steam-pretreated Lespedeza was found to have the most efficient hydrolysis capability to this specific substrate .
	manualset3
240181	4	421945	7	NULL	NULL	0	NULL	specific substrate	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cellulase from steam-pretreated Lespedeza was found to have the most efficient hydrolysis capability to this specific substrate .
	manualset3
240182	1	421946	7	NULL	NULL	0	NULL	PAR ( 1 ) activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PAR ( 1 ) activation appears to rapidly induce transient Galphai1 activation ( t ( 1/2 ) = 4.13 s ) but late and stable recruitment of Galpha12 ( t ( 1/2 ) = 8.8 min ) in parallel with beta-arrestin 1 ( t ( 1/2 ) = 7.5 min ) .
	manualset3
240183	2	421946	7	NULL	NULL	0	NULL	Galphai1 activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PAR ( 1 ) activation appears to rapidly induce transient Galphai1 activation ( t ( 1/2 ) = 4.13 s ) but late and stable recruitment of Galpha12 ( t ( 1/2 ) = 8.8 min ) in parallel with beta-arrestin 1 ( t ( 1/2 ) = 7.5 min ) .
	manualset3
240184	3	421946	7	NULL	NULL	0	NULL	( t ( 1/2 ) = 4.13 s )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PAR ( 1 ) activation appears to rapidly induce transient Galphai1 activation ( t ( 1/2 ) = 4.13 s ) but late and stable recruitment of Galpha12 ( t ( 1/2 ) = 8.8 min ) in parallel with beta-arrestin 1 ( t ( 1/2 ) = 7.5 min ) .
	manualset3
240185	4	421946	7	NULL	NULL	0	NULL	stable recruitment	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	PAR ( 1 ) activation appears to rapidly induce transient Galphai1 activation ( t ( 1/2 ) = 4.13 s ) but late and stable recruitment of Galpha12 ( t ( 1/2 ) = 8.8 min ) in parallel with beta-arrestin 1 ( t ( 1/2 ) = 7.5 min ) .
	manualset3
240186	5	421946	7	NULL	NULL	0	NULL	Galpha12	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PAR ( 1 ) activation appears to rapidly induce transient Galphai1 activation ( t ( 1/2 ) = 4.13 s ) but late and stable recruitment of Galpha12 ( t ( 1/2 ) = 8.8 min ) in parallel with beta-arrestin 1 ( t ( 1/2 ) = 7.5 min ) .
	manualset3
240187	6	421946	7	NULL	NULL	0	NULL	( t ( 1/2 ) = 8.8 min )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PAR ( 1 ) activation appears to rapidly induce transient Galphai1 activation ( t ( 1/2 ) = 4.13 s ) but late and stable recruitment of Galpha12 ( t ( 1/2 ) = 8.8 min ) in parallel with beta-arrestin 1 ( t ( 1/2 ) = 7.5 min ) .
	manualset3
240188	7	421946	7	NULL	NULL	0	NULL	beta-arrestin 1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	PAR ( 1 ) activation appears to rapidly induce transient Galphai1 activation ( t ( 1/2 ) = 4.13 s ) but late and stable recruitment of Galpha12 ( t ( 1/2 ) = 8.8 min ) in parallel with beta-arrestin 1 ( t ( 1/2 ) = 7.5 min ) .
	manualset3
240189	8	421946	7	NULL	NULL	0	NULL	( t ( 1/2 ) = 7.5 min )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	PAR ( 1 ) activation appears to rapidly induce transient Galphai1 activation ( t ( 1/2 ) = 4.13 s ) but late and stable recruitment of Galpha12 ( t ( 1/2 ) = 8.8 min ) in parallel with beta-arrestin 1 ( t ( 1/2 ) = 7.5 min ) .
	manualset3
240190	1	421947	7	NULL	NULL	0	NULL	alpha-interferon ( natural type )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We began to give alpha-interferon ( natural type ) , she had an attack of tonic clonic convulsion ( like grand mal attack ) .
	manualset3
240191	3	421947	7	NULL	NULL	NULL	NULL	tonic clonic convulsion 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We began to give alpha-interferon ( natural type ) , she had an attack of tonic clonic convulsion ( like grand mal attack ) .
	manualset3
240192	4	421947	7	NULL	NULL	0	NULL	 grand mal attack	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We began to give alpha-interferon ( natural type ) , she had an attack of tonic clonic convulsion ( like grand mal attack ) .
	manualset3
240193	2	421947	7	NULL	NULL	0	NULL	attack	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We began to give alpha-interferon ( natural type ) , she had an attack of tonic clonic convulsion ( like grand mal attack ) .
	manualset3
240194	1	421948	7	NULL	NULL	0	NULL	 drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In both instances the drug has to reach the enteric nervous system or the enterocyte , either via the blood or from the lumen , in sufficient concentrations to affect the mediators that regulate motility and fluid transport .
	manualset3
240195	2	421948	7	NULL	NULL	0	NULL	enteric nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In both instances the drug has to reach the enteric nervous system or the enterocyte , either via the blood or from the lumen , in sufficient concentrations to affect the mediators that regulate motility and fluid transport .
	manualset3
240196	3	421948	7	NULL	NULL	0	NULL	enterocyte	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In both instances the drug has to reach the enteric nervous system or the enterocyte , either via the blood or from the lumen , in sufficient concentrations to affect the mediators that regulate motility and fluid transport .
	manualset3
240197	4	421948	7	NULL	NULL	0	NULL	blood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In both instances the drug has to reach the enteric nervous system or the enterocyte , either via the blood or from the lumen , in sufficient concentrations to affect the mediators that regulate motility and fluid transport .
	manualset3
240198	5	421948	7	NULL	NULL	0	NULL	lumen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In both instances the drug has to reach the enteric nervous system or the enterocyte , either via the blood or from the lumen , in sufficient concentrations to affect the mediators that regulate motility and fluid transport .
	manualset3
240199	6	421948	7	NULL	NULL	0	NULL	 concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In both instances the drug has to reach the enteric nervous system or the enterocyte , either via the blood or from the lumen , in sufficient concentrations to affect the mediators that regulate motility and fluid transport .
	manualset3
240200	7	421948	7	NULL	NULL	0	NULL	mediators	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In both instances the drug has to reach the enteric nervous system or the enterocyte , either via the blood or from the lumen , in sufficient concentrations to affect the mediators that regulate motility and fluid transport .
	manualset3
240201	8	421948	7	NULL	NULL	0	NULL	motility	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In both instances the drug has to reach the enteric nervous system or the enterocyte , either via the blood or from the lumen , in sufficient concentrations to affect the mediators that regulate motility and fluid transport .
	manualset3
240202	9	421948	7	NULL	NULL	0	NULL	fluid transport 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In both instances the drug has to reach the enteric nervous system or the enterocyte , either via the blood or from the lumen , in sufficient concentrations to affect the mediators that regulate motility and fluid transport .
	manualset3
240203	1	421949	7	NULL	NULL	NULL	NULL	Chemotaxonomic analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Chemotaxonomic analysis showed a combination of ester-linked 3-OH 10 : 0 , 12 : 1 and amide-linked 3-oxo 14 : 0 ( or 3-OH 14 : 1 ) and 3-OH 14 : 0 fatty acids , which appears to be a unique feature of strains Hel 10 ( T ) and Hel 26 within this subsection of the 2-subclass of the Proteobacteria .
	manualset3
240204	2	421949	7	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Chemotaxonomic analysis showed a combination of ester-linked 3-OH 10 : 0 , 12 : 1 and amide-linked 3-oxo 14 : 0 ( or 3-OH 14 : 1 ) and 3-OH 14 : 0 fatty acids , which appears to be a unique feature of strains Hel 10 ( T ) and Hel 26 within this subsection of the 2-subclass of the Proteobacteria .
	manualset3
240205	3	421949	7	NULL	NULL	NULL	NULL	ester-linked 3-OH 10 : 0 , 12 : 1	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Chemotaxonomic analysis showed a combination of ester-linked 3-OH 10 : 0 , 12 : 1 and amide-linked 3-oxo 14 : 0 ( or 3-OH 14 : 1 ) and 3-OH 14 : 0 fatty acids , which appears to be a unique feature of strains Hel 10 ( T ) and Hel 26 within this subsection of the 2-subclass of the Proteobacteria .
	manualset3
240206	4	421949	7	NULL	NULL	0	NULL	amide-linked 3-oxo 14 : 0 ( or 3-OH 14 : 1 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Chemotaxonomic analysis showed a combination of ester-linked 3-OH 10 : 0 , 12 : 1 and amide-linked 3-oxo 14 : 0 ( or 3-OH 14 : 1 ) and 3-OH 14 : 0 fatty acids , which appears to be a unique feature of strains Hel 10 ( T ) and Hel 26 within this subsection of the 2-subclass of the Proteobacteria .
	manualset3
240207	5	421949	7	NULL	NULL	0	NULL	3-OH 14 : 0 fatty acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Chemotaxonomic analysis showed a combination of ester-linked 3-OH 10 : 0 , 12 : 1 and amide-linked 3-oxo 14 : 0 ( or 3-OH 14 : 1 ) and 3-OH 14 : 0 fatty acids , which appears to be a unique feature of strains Hel 10 ( T ) and Hel 26 within this subsection of the 2-subclass of the Proteobacteria .
	manualset3
240208	6	421949	7	NULL	NULL	0	NULL	strains Hel 10 ( T ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Chemotaxonomic analysis showed a combination of ester-linked 3-OH 10 : 0 , 12 : 1 and amide-linked 3-oxo 14 : 0 ( or 3-OH 14 : 1 ) and 3-OH 14 : 0 fatty acids , which appears to be a unique feature of strains Hel 10 ( T ) and Hel 26 within this subsection of the 2-subclass of the Proteobacteria .
	manualset3
240209	7	421949	7	NULL	NULL	0	NULL	Hel 26	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Chemotaxonomic analysis showed a combination of ester-linked 3-OH 10 : 0 , 12 : 1 and amide-linked 3-oxo 14 : 0 ( or 3-OH 14 : 1 ) and 3-OH 14 : 0 fatty acids , which appears to be a unique feature of strains Hel 10 ( T ) and Hel 26 within this subsection of the 2-subclass of the Proteobacteria .
	manualset3
240210	8	421949	7	NULL	NULL	0	NULL	subsection	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Chemotaxonomic analysis showed a combination of ester-linked 3-OH 10 : 0 , 12 : 1 and amide-linked 3-oxo 14 : 0 ( or 3-OH 14 : 1 ) and 3-OH 14 : 0 fatty acids , which appears to be a unique feature of strains Hel 10 ( T ) and Hel 26 within this subsection of the 2-subclass of the Proteobacteria .
	manualset3
240211	9	421949	7	NULL	NULL	0	NULL	 2-subclass	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Chemotaxonomic analysis showed a combination of ester-linked 3-OH 10 : 0 , 12 : 1 and amide-linked 3-oxo 14 : 0 ( or 3-OH 14 : 1 ) and 3-OH 14 : 0 fatty acids , which appears to be a unique feature of strains Hel 10 ( T ) and Hel 26 within this subsection of the 2-subclass of the Proteobacteria .
	manualset3
240212	10	421949	7	NULL	NULL	0	NULL	Proteobacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Chemotaxonomic analysis showed a combination of ester-linked 3-OH 10 : 0 , 12 : 1 and amide-linked 3-oxo 14 : 0 ( or 3-OH 14 : 1 ) and 3-OH 14 : 0 fatty acids , which appears to be a unique feature of strains Hel 10 ( T ) and Hel 26 within this subsection of the 2-subclass of the Proteobacteria .
	manualset3
240213	1	421950	7	NULL	NULL	0	NULL	Differential regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential regulation of the nocturnal and diurnal prolactin surges in pregnant rats revealed by dopamine receptor antagonism .
	manualset3
240214	2	421950	7	NULL	NULL	0	NULL	nocturnal prolactin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential regulation of the nocturnal and diurnal prolactin surges in pregnant rats revealed by dopamine receptor antagonism .
	manualset3
240215	3	421950	7	NULL	NULL	0	NULL	diurnal prolactin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential regulation of the nocturnal and diurnal prolactin surges in pregnant rats revealed by dopamine receptor antagonism .
	manualset3
240216	4	421950	7	NULL	NULL	0	NULL	pregnant rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential regulation of the nocturnal and diurnal prolactin surges in pregnant rats revealed by dopamine receptor antagonism .
	manualset3
240217	5	421950	7	NULL	NULL	0	NULL	 dopamine receptor antagonism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential regulation of the nocturnal and diurnal prolactin surges in pregnant rats revealed by dopamine receptor antagonism .
	manualset3
240218	1	421951	7	NULL	NULL	0	NULL	20 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 20 patients ( 45 % ) , the initial elicited paresthesia was to the shoulder , whereas in 25 patients ( 55 % ) , the first paresthesia was reported as distal to the shoulder .
	manualset3
240219	2	421951	7	NULL	NULL	0	NULL	45 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 20 patients ( 45 % ) , the initial elicited paresthesia was to the shoulder , whereas in 25 patients ( 55 % ) , the first paresthesia was reported as distal to the shoulder .
	manualset3
240220	3	421951	7	NULL	NULL	0	NULL	initial elicited paresthesia 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In 20 patients ( 45 % ) , the initial elicited paresthesia was to the shoulder , whereas in 25 patients ( 55 % ) , the first paresthesia was reported as distal to the shoulder .
	manualset3
240221	4	421951	7	NULL	NULL	0	NULL	shoulder	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In 20 patients ( 45 % ) , the initial elicited paresthesia was to the shoulder , whereas in 25 patients ( 55 % ) , the first paresthesia was reported as distal to the shoulder .
	manualset3
240222	5	421951	7	NULL	NULL	0	NULL	25 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In 20 patients ( 45 % ) , the initial elicited paresthesia was to the shoulder , whereas in 25 patients ( 55 % ) , the first paresthesia was reported as distal to the shoulder .
	manualset3
240223	6	421951	7	NULL	NULL	0	NULL	55 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In 20 patients ( 45 % ) , the initial elicited paresthesia was to the shoulder , whereas in 25 patients ( 55 % ) , the first paresthesia was reported as distal to the shoulder .
	manualset3
240224	7	421951	7	NULL	NULL	0	NULL	 first paresthesia	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In 20 patients ( 45 % ) , the initial elicited paresthesia was to the shoulder , whereas in 25 patients ( 55 % ) , the first paresthesia was reported as distal to the shoulder .
	manualset3
240225	8	421951	7	NULL	NULL	0	NULL	 distal	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In 20 patients ( 45 % ) , the initial elicited paresthesia was to the shoulder , whereas in 25 patients ( 55 % ) , the first paresthesia was reported as distal to the shoulder .
	manualset3
240226	9	421951	7	NULL	NULL	0	NULL	shoulder	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In 20 patients ( 45 % ) , the initial elicited paresthesia was to the shoulder , whereas in 25 patients ( 55 % ) , the first paresthesia was reported as distal to the shoulder .
	manualset3
240227	1	421952	7	NULL	NULL	0	NULL	electron opaque body	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	An electron opaque body apparently links and anchors all anterior spermatozoid components .
	manualset3
240228	2	421952	7	NULL	NULL	0	NULL	anterior spermatozoid components	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	An electron opaque body apparently links and anchors all anterior spermatozoid components .
	manualset3
240804	1	421953	7	NULL	NULL	0	NULL	three phosphatidylethanolamines ( PEs )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The three phosphatidylethanolamines ( PEs ) were dipetroselinoyl-PE , dioleoyl-PE , and divaccenoyl-PE , which have double bonds in positions 6 , 9 , and 11 , respectively .
	manualset3
240809	2	421953	7	NULL	NULL	0	NULL	dipetroselinoyl-PE	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The three phosphatidylethanolamines ( PEs ) were dipetroselinoyl-PE , dioleoyl-PE , and divaccenoyl-PE , which have double bonds in positions 6 , 9 , and 11 , respectively .
	manualset3
240813	3	421953	7	NULL	NULL	0	NULL	dioleoyl-PE	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The three phosphatidylethanolamines ( PEs ) were dipetroselinoyl-PE , dioleoyl-PE , and divaccenoyl-PE , which have double bonds in positions 6 , 9 , and 11 , respectively .
	manualset3
240814	4	421953	7	NULL	NULL	0	NULL	divaccenoyl-PE	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The three phosphatidylethanolamines ( PEs ) were dipetroselinoyl-PE , dioleoyl-PE , and divaccenoyl-PE , which have double bonds in positions 6 , 9 , and 11 , respectively .
	manualset3
240816	5	421953	7	NULL	NULL	0	NULL	double bonds	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The three phosphatidylethanolamines ( PEs ) were dipetroselinoyl-PE , dioleoyl-PE , and divaccenoyl-PE , which have double bonds in positions 6 , 9 , and 11 , respectively .
	manualset3
240819	6	421953	7	NULL	NULL	0	NULL	positions 6	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The three phosphatidylethanolamines ( PEs ) were dipetroselinoyl-PE , dioleoyl-PE , and divaccenoyl-PE , which have double bonds in positions 6 , 9 , and 11 , respectively .
	manualset3
240820	7	421953	7	NULL	NULL	0	NULL	positions 9	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The three phosphatidylethanolamines ( PEs ) were dipetroselinoyl-PE , dioleoyl-PE , and divaccenoyl-PE , which have double bonds in positions 6 , 9 , and 11 , respectively .
	manualset3
240821	8	421953	7	NULL	NULL	0	NULL	positions 11	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The three phosphatidylethanolamines ( PEs ) were dipetroselinoyl-PE , dioleoyl-PE , and divaccenoyl-PE , which have double bonds in positions 6 , 9 , and 11 , respectively .
	manualset3
240960	1	421954	7	NULL	NULL	0	NULL	parent	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , we examined the influence of parent of origin on expression of 25 murine 22q11 orthologs in the developing and mature CNS using single nucleotide polymorphism ( SNP ) - based analysis in interspecific crosses and quantification of mRNA in a murine model of 22q11DS .
	manualset3
240963	2	421954	7	NULL	NULL	0	NULL	origin	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , we examined the influence of parent of origin on expression of 25 murine 22q11 orthologs in the developing and mature CNS using single nucleotide polymorphism ( SNP ) - based analysis in interspecific crosses and quantification of mRNA in a murine model of 22q11DS .
	manualset3
240964	3	421954	7	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , we examined the influence of parent of origin on expression of 25 murine 22q11 orthologs in the developing and mature CNS using single nucleotide polymorphism ( SNP ) - based analysis in interspecific crosses and quantification of mRNA in a murine model of 22q11DS .
	manualset3
240965	4	421954	7	NULL	NULL	0	NULL	25 murine 22q11 orthologs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , we examined the influence of parent of origin on expression of 25 murine 22q11 orthologs in the developing and mature CNS using single nucleotide polymorphism ( SNP ) - based analysis in interspecific crosses and quantification of mRNA in a murine model of 22q11DS .
	manualset3
240967	5	421954	7	NULL	NULL	0	NULL	mature CNS	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , we examined the influence of parent of origin on expression of 25 murine 22q11 orthologs in the developing and mature CNS using single nucleotide polymorphism ( SNP ) - based analysis in interspecific crosses and quantification of mRNA in a murine model of 22q11DS .
	manualset3
240969	6	421954	7	NULL	NULL	0	NULL	single nucleotide polymorphism ( SNP ) - based analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , we examined the influence of parent of origin on expression of 25 murine 22q11 orthologs in the developing and mature CNS using single nucleotide polymorphism ( SNP ) - based analysis in interspecific crosses and quantification of mRNA in a murine model of 22q11DS .
	manualset3
240970	7	421954	7	NULL	NULL	0	NULL	interspecific crosses	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , we examined the influence of parent of origin on expression of 25 murine 22q11 orthologs in the developing and mature CNS using single nucleotide polymorphism ( SNP ) - based analysis in interspecific crosses and quantification of mRNA in a murine model of 22q11DS .
	manualset3
240971	8	421954	7	NULL	NULL	0	NULL	quantification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , we examined the influence of parent of origin on expression of 25 murine 22q11 orthologs in the developing and mature CNS using single nucleotide polymorphism ( SNP ) - based analysis in interspecific crosses and quantification of mRNA in a murine model of 22q11DS .
	manualset3
240972	9	421954	7	NULL	NULL	0	NULL	mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , we examined the influence of parent of origin on expression of 25 murine 22q11 orthologs in the developing and mature CNS using single nucleotide polymorphism ( SNP ) - based analysis in interspecific crosses and quantification of mRNA in a murine model of 22q11DS .
	manualset3
240973	10	421954	7	NULL	NULL	0	NULL	murine model	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , we examined the influence of parent of origin on expression of 25 murine 22q11 orthologs in the developing and mature CNS using single nucleotide polymorphism ( SNP ) - based analysis in interspecific crosses and quantification of mRNA in a murine model of 22q11DS .
	manualset3
240974	11	421954	7	NULL	NULL	0	NULL	22q11DS	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , we examined the influence of parent of origin on expression of 25 murine 22q11 orthologs in the developing and mature CNS using single nucleotide polymorphism ( SNP ) - based analysis in interspecific crosses and quantification of mRNA in a murine model of 22q11DS .
	manualset3
240975	12	421954	7	NULL	NULL	0	NULL	influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Accordingly , we examined the influence of parent of origin on expression of 25 murine 22q11 orthologs in the developing and mature CNS using single nucleotide polymorphism ( SNP ) - based analysis in interspecific crosses and quantification of mRNA in a murine model of 22q11DS .
	manualset3
240976	1	421955	7	NULL	NULL	0	NULL	general review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	A general review of anomalies of hepatic morphology and their clinical implications .
	manualset3
240977	2	421955	7	NULL	NULL	NULL	NULL	anomalies	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A general review of anomalies of hepatic morphology and their clinical implications .
	manualset3
240981	3	421955	7	NULL	NULL	0	NULL	hepatic morphology 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A general review of anomalies of hepatic morphology and their clinical implications .
	manualset3
240982	4	421955	7	NULL	NULL	0	NULL	clinical implications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A general review of anomalies of hepatic morphology and their clinical implications .
	manualset3
240983	1	421956	7	NULL	NULL	0	NULL	21 cases 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Only 21 cases were determined to be Sudden Infant Death Syndrome ( SIDS ) , which is consistent with the continuous decline of SIDS death in Maryland since 1994 .
	manualset3
240984	2	421956	7	NULL	NULL	0	NULL	Sudden Infant Death Syndrome ( SIDS )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Only 21 cases were determined to be Sudden Infant Death Syndrome ( SIDS ) , which is consistent with the continuous decline of SIDS death in Maryland since 1994 .
	manualset3
240985	3	421956	7	NULL	NULL	0	NULL	continuous decline	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Only 21 cases were determined to be Sudden Infant Death Syndrome ( SIDS ) , which is consistent with the continuous decline of SIDS death in Maryland since 1994 .
	manualset3
240987	4	421956	7	NULL	NULL	0	NULL	SIDS death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Only 21 cases were determined to be Sudden Infant Death Syndrome ( SIDS ) , which is consistent with the continuous decline of SIDS death in Maryland since 1994 .
	manualset3
240989	5	421956	7	NULL	NULL	0	NULL	Maryland	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Only 21 cases were determined to be Sudden Infant Death Syndrome ( SIDS ) , which is consistent with the continuous decline of SIDS death in Maryland since 1994 .
	manualset3
240990	6	421956	7	NULL	NULL	0	NULL	1994	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Only 21 cases were determined to be Sudden Infant Death Syndrome ( SIDS ) , which is consistent with the continuous decline of SIDS death in Maryland since 1994 .
	manualset3
241003	1	421957	7	NULL	NULL	0	NULL	Phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation of tau at both Thr 231 and Ser 262 is required for maximal inhibition of its binding to microtubules .
	manualset3
241005	2	421957	7	NULL	NULL	0	NULL	 tau	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation of tau at both Thr 231 and Ser 262 is required for maximal inhibition of its binding to microtubules .
	manualset3
241006	3	421957	7	NULL	NULL	0	NULL	Thr 231	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation of tau at both Thr 231 and Ser 262 is required for maximal inhibition of its binding to microtubules .
	manualset3
241008	4	421957	7	NULL	NULL	0	NULL	Ser 262 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation of tau at both Thr 231 and Ser 262 is required for maximal inhibition of its binding to microtubules .
	manualset3
241010	5	421957	7	NULL	NULL	0	NULL	maximal inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation of tau at both Thr 231 and Ser 262 is required for maximal inhibition of its binding to microtubules .
	manualset3
241012	6	421957	7	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation of tau at both Thr 231 and Ser 262 is required for maximal inhibition of its binding to microtubules .
	manualset3
241013	7	421957	7	NULL	NULL	0	NULL	microtubules	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Phosphorylation of tau at both Thr 231 and Ser 262 is required for maximal inhibition of its binding to microtubules .
	manualset3
241015	1	421958	7	NULL	NULL	0	NULL	adequate passage	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An adequate passage of tubes was verified in 12 cases through pregnancy , while only in one case HSG was applied , showing a spontaneous recanalization of the right tube .
	manualset3
241016	2	421958	7	NULL	NULL	0	NULL	tubes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An adequate passage of tubes was verified in 12 cases through pregnancy , while only in one case HSG was applied , showing a spontaneous recanalization of the right tube .
	manualset3
241017	3	421958	7	NULL	NULL	0	NULL	12 cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An adequate passage of tubes was verified in 12 cases through pregnancy , while only in one case HSG was applied , showing a spontaneous recanalization of the right tube .
	manualset3
241018	4	421958	7	NULL	NULL	0	NULL	pregnancy 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An adequate passage of tubes was verified in 12 cases through pregnancy , while only in one case HSG was applied , showing a spontaneous recanalization of the right tube .
	manualset3
241021	5	421958	7	NULL	NULL	0	NULL	one case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An adequate passage of tubes was verified in 12 cases through pregnancy , while only in one case HSG was applied , showing a spontaneous recanalization of the right tube .
	manualset3
241024	6	421958	7	NULL	NULL	0	NULL	HSG	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An adequate passage of tubes was verified in 12 cases through pregnancy , while only in one case HSG was applied , showing a spontaneous recanalization of the right tube .
	manualset3
241025	7	421958	7	NULL	NULL	0	NULL	spontaneous recanalization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An adequate passage of tubes was verified in 12 cases through pregnancy , while only in one case HSG was applied , showing a spontaneous recanalization of the right tube .
	manualset3
241026	8	421958	7	NULL	NULL	0	NULL	right tube	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An adequate passage of tubes was verified in 12 cases through pregnancy , while only in one case HSG was applied , showing a spontaneous recanalization of the right tube .
	manualset3
241034	1	421959	7	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the focal points in the present article is how a localized increased tissue pressure may persist in the inflamed area without a circumferential spread to the rest of the pulp .
	manualset3
241035	2	421959	7	NULL	NULL	0	NULL	focal points	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the focal points in the present article is how a localized increased tissue pressure may persist in the inflamed area without a circumferential spread to the rest of the pulp .
	manualset3
241037	3	421959	7	NULL	NULL	0	NULL	 article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the focal points in the present article is how a localized increased tissue pressure may persist in the inflamed area without a circumferential spread to the rest of the pulp .
	manualset3
241038	4	421959	7	NULL	NULL	0	NULL	 tissue pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the focal points in the present article is how a localized increased tissue pressure may persist in the inflamed area without a circumferential spread to the rest of the pulp .
	manualset3
241039	5	421959	7	NULL	NULL	0	NULL	inflamed area	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the focal points in the present article is how a localized increased tissue pressure may persist in the inflamed area without a circumferential spread to the rest of the pulp .
	manualset3
241040	6	421959	7	NULL	NULL	NULL	NULL	 rest of the pulp	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	One of the focal points in the present article is how a localized increased tissue pressure may persist in the inflamed area without a circumferential spread to the rest of the pulp .
	manualset3
241041	1	421960	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that the eyelids of mice had both alpha-1 and alpha-2 adrenoceptors .
	manualset3
241042	2	421960	7	NULL	NULL	0	NULL	eyelids	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that the eyelids of mice had both alpha-1 and alpha-2 adrenoceptors .
	manualset3
241043	3	421960	7	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that the eyelids of mice had both alpha-1 and alpha-2 adrenoceptors .
	manualset3
241044	4	421960	7	NULL	NULL	NULL	NULL	alpha-1 adrenoceptors	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results suggested that the eyelids of mice had both alpha-1 and alpha-2 adrenoceptors .
	manualset3
241045	5	421960	7	NULL	NULL	0	NULL	 alpha-2 adrenoceptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These results suggested that the eyelids of mice had both alpha-1 and alpha-2 adrenoceptors .
	manualset3
241047	1	421961	7	NULL	NULL	0	NULL	Change	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Change of attitude is needed .
	manualset3
241049	2	421961	7	NULL	NULL	0	NULL	attitude	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Change of attitude is needed .
	manualset3
241052	1	421962	7	NULL	NULL	0	NULL	cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	All cases were diagnosed by computed tomography and none underwent surgery .
	manualset3
241053	2	421962	7	NULL	NULL	0	NULL	computed tomography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All cases were diagnosed by computed tomography and none underwent surgery .
	manualset3
241055	3	421962	7	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	All cases were diagnosed by computed tomography and none underwent surgery .
	manualset3
241061	1	421963	7	NULL	NULL	0	NULL	21-year-old woman	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	A 21-year-old woman with a hepatic mass after treatment for amenorrhea .
	manualset3
241063	2	421963	7	NULL	NULL	0	NULL	hepatic mass	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 21-year-old woman with a hepatic mass after treatment for amenorrhea .
	manualset3
241065	3	421963	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A 21-year-old woman with a hepatic mass after treatment for amenorrhea .
	manualset3
241066	4	421963	7	NULL	NULL	0	NULL	amenorrhea	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 21-year-old woman with a hepatic mass after treatment for amenorrhea .
	manualset3
241069	1	421964	7	NULL	NULL	0	NULL	Human keratinocytes ( HK )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Human keratinocytes ( HK ) and fibroblasts ( HF ) derived from foreskins , were further cultured during 24 h in defined medium , supplemented or not with the selected growth factors , EGF and TGF-beta1 , respectively , before receiving the addition of either IL-4 or IFN-gamma during 24 and 48 h. In basal conditions , fibroblasts produced smaller amounts of VEGF than keratinocytes ; the addition of growth factors to the skin cells induced a drastic increase of VEGF secretion .
	manualset3
241070	2	421964	7	NULL	NULL	0	NULL	fibroblasts ( HF ) 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Human keratinocytes ( HK ) and fibroblasts ( HF ) derived from foreskins , were further cultured during 24 h in defined medium , supplemented or not with the selected growth factors , EGF and TGF-beta1 , respectively , before receiving the addition of either IL-4 or IFN-gamma during 24 and 48 h. In basal conditions , fibroblasts produced smaller amounts of VEGF than keratinocytes ; the addition of growth factors to the skin cells induced a drastic increase of VEGF secretion .
	manualset3
241073	3	421964	7	NULL	NULL	0	NULL	foreskins	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Human keratinocytes ( HK ) and fibroblasts ( HF ) derived from foreskins , were further cultured during 24 h in defined medium , supplemented or not with the selected growth factors , EGF and TGF-beta1 , respectively , before receiving the addition of either IL-4 or IFN-gamma during 24 and 48 h. In basal conditions , fibroblasts produced smaller amounts of VEGF than keratinocytes ; the addition of growth factors to the skin cells induced a drastic increase of VEGF secretion .
	manualset3
241074	4	421964	7	NULL	NULL	0	NULL	 24 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Human keratinocytes ( HK ) and fibroblasts ( HF ) derived from foreskins , were further cultured during 24 h in defined medium , supplemented or not with the selected growth factors , EGF and TGF-beta1 , respectively , before receiving the addition of either IL-4 or IFN-gamma during 24 and 48 h. In basal conditions , fibroblasts produced smaller amounts of VEGF than keratinocytes ; the addition of growth factors to the skin cells induced a drastic increase of VEGF secretion .
	manualset3
241075	5	421964	7	NULL	NULL	0	NULL	defined medium	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Human keratinocytes ( HK ) and fibroblasts ( HF ) derived from foreskins , were further cultured during 24 h in defined medium , supplemented or not with the selected growth factors , EGF and TGF-beta1 , respectively , before receiving the addition of either IL-4 or IFN-gamma during 24 and 48 h. In basal conditions , fibroblasts produced smaller amounts of VEGF than keratinocytes ; the addition of growth factors to the skin cells induced a drastic increase of VEGF secretion .
	manualset3
241077	6	421964	7	NULL	NULL	0	NULL	growth factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Human keratinocytes ( HK ) and fibroblasts ( HF ) derived from foreskins , were further cultured during 24 h in defined medium , supplemented or not with the selected growth factors , EGF and TGF-beta1 , respectively , before receiving the addition of either IL-4 or IFN-gamma during 24 and 48 h. In basal conditions , fibroblasts produced smaller amounts of VEGF than keratinocytes ; the addition of growth factors to the skin cells induced a drastic increase of VEGF secretion .
	manualset3
241079	7	421964	7	NULL	NULL	0	NULL	EGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human keratinocytes ( HK ) and fibroblasts ( HF ) derived from foreskins , were further cultured during 24 h in defined medium , supplemented or not with the selected growth factors , EGF and TGF-beta1 , respectively , before receiving the addition of either IL-4 or IFN-gamma during 24 and 48 h. In basal conditions , fibroblasts produced smaller amounts of VEGF than keratinocytes ; the addition of growth factors to the skin cells induced a drastic increase of VEGF secretion .
	manualset3
241080	8	421964	7	NULL	NULL	0	NULL	TGF-beta1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human keratinocytes ( HK ) and fibroblasts ( HF ) derived from foreskins , were further cultured during 24 h in defined medium , supplemented or not with the selected growth factors , EGF and TGF-beta1 , respectively , before receiving the addition of either IL-4 or IFN-gamma during 24 and 48 h. In basal conditions , fibroblasts produced smaller amounts of VEGF than keratinocytes ; the addition of growth factors to the skin cells induced a drastic increase of VEGF secretion .
	manualset3
241081	9	421964	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Human keratinocytes ( HK ) and fibroblasts ( HF ) derived from foreskins , were further cultured during 24 h in defined medium , supplemented or not with the selected growth factors , EGF and TGF-beta1 , respectively , before receiving the addition of either IL-4 or IFN-gamma during 24 and 48 h. In basal conditions , fibroblasts produced smaller amounts of VEGF than keratinocytes ; the addition of growth factors to the skin cells induced a drastic increase of VEGF secretion .
	manualset3
241082	10	421964	7	NULL	NULL	0	NULL	IL-4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human keratinocytes ( HK ) and fibroblasts ( HF ) derived from foreskins , were further cultured during 24 h in defined medium , supplemented or not with the selected growth factors , EGF and TGF-beta1 , respectively , before receiving the addition of either IL-4 or IFN-gamma during 24 and 48 h. In basal conditions , fibroblasts produced smaller amounts of VEGF than keratinocytes ; the addition of growth factors to the skin cells induced a drastic increase of VEGF secretion .
	manualset3
241083	11	421964	7	NULL	NULL	0	NULL	IFN-gamma 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human keratinocytes ( HK ) and fibroblasts ( HF ) derived from foreskins , were further cultured during 24 h in defined medium , supplemented or not with the selected growth factors , EGF and TGF-beta1 , respectively , before receiving the addition of either IL-4 or IFN-gamma during 24 and 48 h. In basal conditions , fibroblasts produced smaller amounts of VEGF than keratinocytes ; the addition of growth factors to the skin cells induced a drastic increase of VEGF secretion .
	manualset3
241084	12	421964	7	NULL	NULL	0	NULL	24h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Human keratinocytes ( HK ) and fibroblasts ( HF ) derived from foreskins , were further cultured during 24 h in defined medium , supplemented or not with the selected growth factors , EGF and TGF-beta1 , respectively , before receiving the addition of either IL-4 or IFN-gamma during 24 and 48 h. In basal conditions , fibroblasts produced smaller amounts of VEGF than keratinocytes ; the addition of growth factors to the skin cells induced a drastic increase of VEGF secretion .
	manualset3
241086	13	421964	7	NULL	NULL	0	NULL	48 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Human keratinocytes ( HK ) and fibroblasts ( HF ) derived from foreskins , were further cultured during 24 h in defined medium , supplemented or not with the selected growth factors , EGF and TGF-beta1 , respectively , before receiving the addition of either IL-4 or IFN-gamma during 24 and 48 h. In basal conditions , fibroblasts produced smaller amounts of VEGF than keratinocytes ; the addition of growth factors to the skin cells induced a drastic increase of VEGF secretion .
	manualset3
241088	14	421964	7	NULL	NULL	0	NULL	basal conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Human keratinocytes ( HK ) and fibroblasts ( HF ) derived from foreskins , were further cultured during 24 h in defined medium , supplemented or not with the selected growth factors , EGF and TGF-beta1 , respectively , before receiving the addition of either IL-4 or IFN-gamma during 24 and 48 h. In basal conditions , fibroblasts produced smaller amounts of VEGF than keratinocytes ; the addition of growth factors to the skin cells induced a drastic increase of VEGF secretion .
	manualset3
241090	15	421964	7	NULL	NULL	0	NULL	fibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Human keratinocytes ( HK ) and fibroblasts ( HF ) derived from foreskins , were further cultured during 24 h in defined medium , supplemented or not with the selected growth factors , EGF and TGF-beta1 , respectively , before receiving the addition of either IL-4 or IFN-gamma during 24 and 48 h. In basal conditions , fibroblasts produced smaller amounts of VEGF than keratinocytes ; the addition of growth factors to the skin cells induced a drastic increase of VEGF secretion .
	manualset3
241092	16	421964	7	NULL	NULL	0	NULL	smaller amounts 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Human keratinocytes ( HK ) and fibroblasts ( HF ) derived from foreskins , were further cultured during 24 h in defined medium , supplemented or not with the selected growth factors , EGF and TGF-beta1 , respectively , before receiving the addition of either IL-4 or IFN-gamma during 24 and 48 h. In basal conditions , fibroblasts produced smaller amounts of VEGF than keratinocytes ; the addition of growth factors to the skin cells induced a drastic increase of VEGF secretion .
	manualset3
241094	17	421964	7	NULL	NULL	0	NULL	VEGF 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Human keratinocytes ( HK ) and fibroblasts ( HF ) derived from foreskins , were further cultured during 24 h in defined medium , supplemented or not with the selected growth factors , EGF and TGF-beta1 , respectively , before receiving the addition of either IL-4 or IFN-gamma during 24 and 48 h. In basal conditions , fibroblasts produced smaller amounts of VEGF than keratinocytes ; the addition of growth factors to the skin cells induced a drastic increase of VEGF secretion .
	manualset3
241095	18	421964	7	NULL	NULL	0	NULL	keratinocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Human keratinocytes ( HK ) and fibroblasts ( HF ) derived from foreskins , were further cultured during 24 h in defined medium , supplemented or not with the selected growth factors , EGF and TGF-beta1 , respectively , before receiving the addition of either IL-4 or IFN-gamma during 24 and 48 h. In basal conditions , fibroblasts produced smaller amounts of VEGF than keratinocytes ; the addition of growth factors to the skin cells induced a drastic increase of VEGF secretion .
	manualset3
241098	19	421964	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Human keratinocytes ( HK ) and fibroblasts ( HF ) derived from foreskins , were further cultured during 24 h in defined medium , supplemented or not with the selected growth factors , EGF and TGF-beta1 , respectively , before receiving the addition of either IL-4 or IFN-gamma during 24 and 48 h. In basal conditions , fibroblasts produced smaller amounts of VEGF than keratinocytes ; the addition of growth factors to the skin cells induced a drastic increase of VEGF secretion .
	manualset3
241100	20	421964	7	NULL	NULL	0	NULL	 growth factors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Human keratinocytes ( HK ) and fibroblasts ( HF ) derived from foreskins , were further cultured during 24 h in defined medium , supplemented or not with the selected growth factors , EGF and TGF-beta1 , respectively , before receiving the addition of either IL-4 or IFN-gamma during 24 and 48 h. In basal conditions , fibroblasts produced smaller amounts of VEGF than keratinocytes ; the addition of growth factors to the skin cells induced a drastic increase of VEGF secretion .
	manualset3
241101	21	421964	7	NULL	NULL	0	NULL	 skin cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Human keratinocytes ( HK ) and fibroblasts ( HF ) derived from foreskins , were further cultured during 24 h in defined medium , supplemented or not with the selected growth factors , EGF and TGF-beta1 , respectively , before receiving the addition of either IL-4 or IFN-gamma during 24 and 48 h. In basal conditions , fibroblasts produced smaller amounts of VEGF than keratinocytes ; the addition of growth factors to the skin cells induced a drastic increase of VEGF secretion .
	manualset3
241103	22	421964	7	NULL	NULL	0	NULL	increase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Human keratinocytes ( HK ) and fibroblasts ( HF ) derived from foreskins , were further cultured during 24 h in defined medium , supplemented or not with the selected growth factors , EGF and TGF-beta1 , respectively , before receiving the addition of either IL-4 or IFN-gamma during 24 and 48 h. In basal conditions , fibroblasts produced smaller amounts of VEGF than keratinocytes ; the addition of growth factors to the skin cells induced a drastic increase of VEGF secretion .
	manualset3
241104	23	421964	7	NULL	NULL	0	NULL	VEGF secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Human keratinocytes ( HK ) and fibroblasts ( HF ) derived from foreskins , were further cultured during 24 h in defined medium , supplemented or not with the selected growth factors , EGF and TGF-beta1 , respectively , before receiving the addition of either IL-4 or IFN-gamma during 24 and 48 h. In basal conditions , fibroblasts produced smaller amounts of VEGF than keratinocytes ; the addition of growth factors to the skin cells induced a drastic increase of VEGF secretion .
	manualset3
241107	1	421965	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients received erythropoietin , and iron was administered intravenously to maintain the hemoglobin level between 10 and 12 mg/dL .
	manualset3
241108	2	421965	7	NULL	NULL	0	NULL	erythropoietin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients received erythropoietin , and iron was administered intravenously to maintain the hemoglobin level between 10 and 12 mg/dL .
	manualset3
241109	3	421965	7	NULL	NULL	0	NULL	iron	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients received erythropoietin , and iron was administered intravenously to maintain the hemoglobin level between 10 and 12 mg/dL .
	manualset3
241110	4	421965	7	NULL	NULL	0	NULL	hemoglobin level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients received erythropoietin , and iron was administered intravenously to maintain the hemoglobin level between 10 and 12 mg/dL .
	manualset3
241111	5	421965	7	NULL	NULL	0	NULL	 10 mg/dL	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients received erythropoietin , and iron was administered intravenously to maintain the hemoglobin level between 10 and 12 mg/dL .
	manualset3
241112	6	421965	7	NULL	NULL	0	NULL	12 mg/dL	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	All patients received erythropoietin , and iron was administered intravenously to maintain the hemoglobin level between 10 and 12 mg/dL .
	manualset3
241113	1	421966	7	NULL	NULL	0	NULL	enantioselective formal total synthesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An enantioselective formal total synthesis of the cytotoxic macrolide ( + ) - aspergillide C has been accomplished from ( S ) - ( - ) - glyceraldehyde acetonide and the Danishefsky-Kitahara diene .
	manualset3
241114	2	421966	7	NULL	NULL	0	NULL	cytotoxic macrolide ( + ) - aspergillide C	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An enantioselective formal total synthesis of the cytotoxic macrolide ( + ) - aspergillide C has been accomplished from ( S ) - ( - ) - glyceraldehyde acetonide and the Danishefsky-Kitahara diene .
	manualset3
241115	3	421966	7	NULL	NULL	0	NULL	( S ) - ( - ) - glyceraldehyde acetonide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An enantioselective formal total synthesis of the cytotoxic macrolide ( + ) - aspergillide C has been accomplished from ( S ) - ( - ) - glyceraldehyde acetonide and the Danishefsky-Kitahara diene .
	manualset3
241116	4	421966	7	NULL	NULL	0	NULL	Danishefsky-Kitahara diene .	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An enantioselective formal total synthesis of the cytotoxic macrolide ( + ) - aspergillide C has been accomplished from ( S ) - ( - ) - glyceraldehyde acetonide and the Danishefsky-Kitahara diene .
	manualset3
241117	1	421967	7	NULL	NULL	0	NULL	chemical shifts	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemical shifts of these peaks were not strongly dependent on the oxidation state of the protein , although relative ratios of line widths of several peaks in the spectra of oxidized and reduced Rd suggested localized conformational changes of the protein as a result of oxidation .
	manualset3
241118	2	421967	7	NULL	NULL	0	NULL	peaks	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemical shifts of these peaks were not strongly dependent on the oxidation state of the protein , although relative ratios of line widths of several peaks in the spectra of oxidized and reduced Rd suggested localized conformational changes of the protein as a result of oxidation .
	manualset3
241119	3	421967	7	NULL	NULL	0	NULL	oxidation state	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemical shifts of these peaks were not strongly dependent on the oxidation state of the protein , although relative ratios of line widths of several peaks in the spectra of oxidized and reduced Rd suggested localized conformational changes of the protein as a result of oxidation .
	manualset3
241120	4	421967	7	NULL	NULL	NULL	NULL	protein	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The chemical shifts of these peaks were not strongly dependent on the oxidation state of the protein , although relative ratios of line widths of several peaks in the spectra of oxidized and reduced Rd suggested localized conformational changes of the protein as a result of oxidation .
	manualset3
241121	5	421967	7	NULL	NULL	0	NULL	relative ratios	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemical shifts of these peaks were not strongly dependent on the oxidation state of the protein , although relative ratios of line widths of several peaks in the spectra of oxidized and reduced Rd suggested localized conformational changes of the protein as a result of oxidation .
	manualset3
241122	6	421967	7	NULL	NULL	0	NULL	line widths	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemical shifts of these peaks were not strongly dependent on the oxidation state of the protein , although relative ratios of line widths of several peaks in the spectra of oxidized and reduced Rd suggested localized conformational changes of the protein as a result of oxidation .
	manualset3
241123	7	421967	7	NULL	NULL	0	NULL	several peaks	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemical shifts of these peaks were not strongly dependent on the oxidation state of the protein , although relative ratios of line widths of several peaks in the spectra of oxidized and reduced Rd suggested localized conformational changes of the protein as a result of oxidation .
	manualset3
241124	8	421967	7	NULL	NULL	0	NULL	spectra 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemical shifts of these peaks were not strongly dependent on the oxidation state of the protein , although relative ratios of line widths of several peaks in the spectra of oxidized and reduced Rd suggested localized conformational changes of the protein as a result of oxidation .
	manualset3
241125	9	421967	7	NULL	NULL	0	NULL	oxidized Rd	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemical shifts of these peaks were not strongly dependent on the oxidation state of the protein , although relative ratios of line widths of several peaks in the spectra of oxidized and reduced Rd suggested localized conformational changes of the protein as a result of oxidation .
	manualset3
241126	10	421967	7	NULL	NULL	0	NULL	reduced Rd	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemical shifts of these peaks were not strongly dependent on the oxidation state of the protein , although relative ratios of line widths of several peaks in the spectra of oxidized and reduced Rd suggested localized conformational changes of the protein as a result of oxidation .
	manualset3
241127	11	421967	7	NULL	NULL	0	NULL	localized conformational changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemical shifts of these peaks were not strongly dependent on the oxidation state of the protein , although relative ratios of line widths of several peaks in the spectra of oxidized and reduced Rd suggested localized conformational changes of the protein as a result of oxidation .
	manualset3
241128	12	421967	7	NULL	NULL	0	NULL	protein	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemical shifts of these peaks were not strongly dependent on the oxidation state of the protein , although relative ratios of line widths of several peaks in the spectra of oxidized and reduced Rd suggested localized conformational changes of the protein as a result of oxidation .
	manualset3
241129	13	421967	7	NULL	NULL	0	NULL	result	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The chemical shifts of these peaks were not strongly dependent on the oxidation state of the protein , although relative ratios of line widths of several peaks in the spectra of oxidized and reduced Rd suggested localized conformational changes of the protein as a result of oxidation .
	manualset3
241130	14	421967	7	NULL	NULL	NULL	NULL	oxidation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The chemical shifts of these peaks were not strongly dependent on the oxidation state of the protein , although relative ratios of line widths of several peaks in the spectra of oxidized and reduced Rd suggested localized conformational changes of the protein as a result of oxidation .
	manualset3
241131	1	421968	7	NULL	NULL	0	NULL	underlying clear layer	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The underlying clear layer does not contain keratohyalin-like granules but has a rich cytoskeleton of intermediate filaments .
	manualset3
241132	2	421968	7	NULL	NULL	0	NULL	 keratohyalin-like granules	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The underlying clear layer does not contain keratohyalin-like granules but has a rich cytoskeleton of intermediate filaments .
	manualset3
241133	3	421968	7	NULL	NULL	0	NULL	rich cytoskeleton of intermediate filaments	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The underlying clear layer does not contain keratohyalin-like granules but has a rich cytoskeleton of intermediate filaments .
	manualset3
241134	1	421969	7	NULL	NULL	NULL	NULL	appreciable change	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There was no appreciable change in the discharge following the NaCl injections into the portal and jugular veins , and the portal glucose responses in the discharge were abolished by transection of the hepatic branch of the vagus nerve .
	manualset3
241135	2	421969	7	NULL	NULL	NULL	NULL	discharge	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There was no appreciable change in the discharge following the NaCl injections into the portal and jugular veins , and the portal glucose responses in the discharge were abolished by transection of the hepatic branch of the vagus nerve .
	manualset3
241136	3	421969	7	NULL	NULL	0	NULL	NaCl injections	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no appreciable change in the discharge following the NaCl injections into the portal and jugular veins , and the portal glucose responses in the discharge were abolished by transection of the hepatic branch of the vagus nerve .
	manualset3
241137	4	421969	7	NULL	NULL	0	NULL	portal veins	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no appreciable change in the discharge following the NaCl injections into the portal and jugular veins , and the portal glucose responses in the discharge were abolished by transection of the hepatic branch of the vagus nerve .
	manualset3
241138	5	421969	7	NULL	NULL	0	NULL	jugular veins	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no appreciable change in the discharge following the NaCl injections into the portal and jugular veins , and the portal glucose responses in the discharge were abolished by transection of the hepatic branch of the vagus nerve .
	manualset3
241139	6	421969	7	NULL	NULL	0	NULL	portal glucose responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no appreciable change in the discharge following the NaCl injections into the portal and jugular veins , and the portal glucose responses in the discharge were abolished by transection of the hepatic branch of the vagus nerve .
	manualset3
241140	7	421969	7	NULL	NULL	NULL	NULL	discharge	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There was no appreciable change in the discharge following the NaCl injections into the portal and jugular veins , and the portal glucose responses in the discharge were abolished by transection of the hepatic branch of the vagus nerve .
	manualset3
241141	8	421969	7	NULL	NULL	0	NULL	transection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no appreciable change in the discharge following the NaCl injections into the portal and jugular veins , and the portal glucose responses in the discharge were abolished by transection of the hepatic branch of the vagus nerve .
	manualset3
241142	9	421969	7	NULL	NULL	NULL	NULL	hepatic branch 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	There was no appreciable change in the discharge following the NaCl injections into the portal and jugular veins , and the portal glucose responses in the discharge were abolished by transection of the hepatic branch of the vagus nerve .
	manualset3
243960	10	421969	7	NULL	NULL	0	NULL	 vagus nerve	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	There was no appreciable change in the discharge following the NaCl injections into the portal and jugular veins , and the portal glucose responses in the discharge were abolished by transection of the hepatic branch of the vagus nerve .
	manualset3
241143	1	421970	7	NULL	NULL	0	NULL	temperature retrieval method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The temperature retrieval method has an uncertainty of less than 2.5 degrees C , resulting in a 0.3 % uncertainty in the correction to be performed .
	manualset3
241144	2	421970	7	NULL	NULL	0	NULL	 2.5 degrees C	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The temperature retrieval method has an uncertainty of less than 2.5 degrees C , resulting in a 0.3 % uncertainty in the correction to be performed .
	manualset3
241145	3	421970	7	NULL	NULL	0	NULL	0.3 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The temperature retrieval method has an uncertainty of less than 2.5 degrees C , resulting in a 0.3 % uncertainty in the correction to be performed .
	manualset3
241146	4	421970	7	NULL	NULL	0	NULL	correction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The temperature retrieval method has an uncertainty of less than 2.5 degrees C , resulting in a 0.3 % uncertainty in the correction to be performed .
	manualset3
241147	1	421971	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of osteocyte autophagy , as detected by immunostaining for LC3 , increased 50 % at the distal femur cortical bone region but not at trabecular bone region at the 1.4 and 2.8 mg/kg/d GC dose levels .
	manualset3
241148	2	421971	7	NULL	NULL	0	NULL	osteocyte autophagy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of osteocyte autophagy , as detected by immunostaining for LC3 , increased 50 % at the distal femur cortical bone region but not at trabecular bone region at the 1.4 and 2.8 mg/kg/d GC dose levels .
	manualset3
241149	3	421971	7	NULL	NULL	0	NULL	immunostaining	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of osteocyte autophagy , as detected by immunostaining for LC3 , increased 50 % at the distal femur cortical bone region but not at trabecular bone region at the 1.4 and 2.8 mg/kg/d GC dose levels .
	manualset3
241150	4	421971	7	NULL	NULL	0	NULL	 LC3 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of osteocyte autophagy , as detected by immunostaining for LC3 , increased 50 % at the distal femur cortical bone region but not at trabecular bone region at the 1.4 and 2.8 mg/kg/d GC dose levels .
	manualset3
241151	5	421971	7	NULL	NULL	0	NULL	50 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of osteocyte autophagy , as detected by immunostaining for LC3 , increased 50 % at the distal femur cortical bone region but not at trabecular bone region at the 1.4 and 2.8 mg/kg/d GC dose levels .
	manualset3
241152	6	421971	7	NULL	NULL	0	NULL	distal femur cortical bone region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of osteocyte autophagy , as detected by immunostaining for LC3 , increased 50 % at the distal femur cortical bone region but not at trabecular bone region at the 1.4 and 2.8 mg/kg/d GC dose levels .
	manualset3
241153	7	421971	7	NULL	NULL	0	NULL	trabecular bone region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of osteocyte autophagy , as detected by immunostaining for LC3 , increased 50 % at the distal femur cortical bone region but not at trabecular bone region at the 1.4 and 2.8 mg/kg/d GC dose levels .
	manualset3
241154	8	421971	7	NULL	NULL	0	NULL	1.4 mg/kg/d GC dose levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of osteocyte autophagy , as detected by immunostaining for LC3 , increased 50 % at the distal femur cortical bone region but not at trabecular bone region at the 1.4 and 2.8 mg/kg/d GC dose levels .
	manualset3
241155	9	421971	7	NULL	NULL	0	NULL	2.8 mg/kg/d GC dose levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The presence of osteocyte autophagy , as detected by immunostaining for LC3 , increased 50 % at the distal femur cortical bone region but not at trabecular bone region at the 1.4 and 2.8 mg/kg/d GC dose levels .
	manualset3
241156	1	421972	7	NULL	NULL	0	NULL	sensitive stages	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The more sensitive stages ( late trophozoites and schizonts ) were better protected by using the freezing program designed for lymphocytes .
	manualset3
241157	2	421972	7	NULL	NULL	NULL	NULL	late trophozoites 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The more sensitive stages ( late trophozoites and schizonts ) were better protected by using the freezing program designed for lymphocytes .
	manualset3
241158	3	421972	7	NULL	NULL	0	NULL	schizonts	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The more sensitive stages ( late trophozoites and schizonts ) were better protected by using the freezing program designed for lymphocytes .
	manualset3
241159	4	421972	7	NULL	NULL	0	NULL	freezing program 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The more sensitive stages ( late trophozoites and schizonts ) were better protected by using the freezing program designed for lymphocytes .
	manualset3
241160	5	421972	7	NULL	NULL	0	NULL	lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The more sensitive stages ( late trophozoites and schizonts ) were better protected by using the freezing program designed for lymphocytes .
	manualset3
241161	1	421973	7	NULL	NULL	0	NULL	endonuclease activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An endonuclease activity in Bacillus subtilis specific for UV-irradiated DNA .
	manualset3
241162	2	421973	7	NULL	NULL	0	NULL	Bacillus subtilis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	An endonuclease activity in Bacillus subtilis specific for UV-irradiated DNA .
	manualset3
241163	3	421973	7	NULL	NULL	0	NULL	UV-irradiated DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	An endonuclease activity in Bacillus subtilis specific for UV-irradiated DNA .
	manualset3
241164	1	421974	7	NULL	NULL	0	NULL	mechanisms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We review the mechanisms of gas exchange , as well as the indications , monitoring and special features of the use HVOF in the neonatal period .
	manualset3
241165	2	421974	7	NULL	NULL	0	NULL	gas exchange	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We review the mechanisms of gas exchange , as well as the indications , monitoring and special features of the use HVOF in the neonatal period .
	manualset3
241166	3	421974	7	NULL	NULL	0	NULL	indications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We review the mechanisms of gas exchange , as well as the indications , monitoring and special features of the use HVOF in the neonatal period .
	manualset3
241168	4	421974	7	NULL	NULL	0	NULL	HVOF	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	We review the mechanisms of gas exchange , as well as the indications , monitoring and special features of the use HVOF in the neonatal period .
	manualset3
241169	5	421974	7	NULL	NULL	0	NULL	neonatal period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	We review the mechanisms of gas exchange , as well as the indications , monitoring and special features of the use HVOF in the neonatal period .
	manualset3
241170	6	421974	7	NULL	NULL	0	NULL	special features	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We review the mechanisms of gas exchange , as well as the indications , monitoring and special features of the use HVOF in the neonatal period .
	manualset3
243961	7	421974	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We review the mechanisms of gas exchange , as well as the indications , monitoring and special features of the use HVOF in the neonatal period .
	manualset3
247390	8	421974	7	NULL	NULL	0	NULL	monitoring	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We review the mechanisms of gas exchange , as well as the indications , monitoring and special features of the use HVOF in the neonatal period .
	manualset3
241171	1	421975	7	NULL	NULL	0	NULL	present studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present studies were designed to investigate the effect of the physiological stimulants bradykinin ( BK ) and 5-hydroxytryptamine ( 5-HT ) , in addition to the influence of the calcium ionophore A23187 , on the source of AA release and 5-lipoxygenation in human neutrophils ( PMNs ) in vitro .
	manualset3
241172	2	421975	7	NULL	NULL	0	NULL	effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present studies were designed to investigate the effect of the physiological stimulants bradykinin ( BK ) and 5-hydroxytryptamine ( 5-HT ) , in addition to the influence of the calcium ionophore A23187 , on the source of AA release and 5-lipoxygenation in human neutrophils ( PMNs ) in vitro .
	manualset3
241173	3	421975	7	NULL	NULL	NULL	NULL	 physiological stimulants	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present studies were designed to investigate the effect of the physiological stimulants bradykinin ( BK ) and 5-hydroxytryptamine ( 5-HT ) , in addition to the influence of the calcium ionophore A23187 , on the source of AA release and 5-lipoxygenation in human neutrophils ( PMNs ) in vitro .
	manualset3
241174	4	421975	7	NULL	NULL	0	NULL	bradykinin ( BK ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present studies were designed to investigate the effect of the physiological stimulants bradykinin ( BK ) and 5-hydroxytryptamine ( 5-HT ) , in addition to the influence of the calcium ionophore A23187 , on the source of AA release and 5-lipoxygenation in human neutrophils ( PMNs ) in vitro .
	manualset3
241175	5	421975	7	NULL	NULL	0	NULL	5-hydroxytryptamine ( 5-HT )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The present studies were designed to investigate the effect of the physiological stimulants bradykinin ( BK ) and 5-hydroxytryptamine ( 5-HT ) , in addition to the influence of the calcium ionophore A23187 , on the source of AA release and 5-lipoxygenation in human neutrophils ( PMNs ) in vitro .
	manualset3
241176	6	421975	7	NULL	NULL	0	NULL	 influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The present studies were designed to investigate the effect of the physiological stimulants bradykinin ( BK ) and 5-hydroxytryptamine ( 5-HT ) , in addition to the influence of the calcium ionophore A23187 , on the source of AA release and 5-lipoxygenation in human neutrophils ( PMNs ) in vitro .
	manualset3
241177	7	421975	7	NULL	NULL	0	NULL	calcium ionophore A23187	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The present studies were designed to investigate the effect of the physiological stimulants bradykinin ( BK ) and 5-hydroxytryptamine ( 5-HT ) , in addition to the influence of the calcium ionophore A23187 , on the source of AA release and 5-lipoxygenation in human neutrophils ( PMNs ) in vitro .
	manualset3
241178	8	421975	7	NULL	NULL	0	NULL	source 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present studies were designed to investigate the effect of the physiological stimulants bradykinin ( BK ) and 5-hydroxytryptamine ( 5-HT ) , in addition to the influence of the calcium ionophore A23187 , on the source of AA release and 5-lipoxygenation in human neutrophils ( PMNs ) in vitro .
	manualset3
241179	9	421975	7	NULL	NULL	0	NULL	AA release 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present studies were designed to investigate the effect of the physiological stimulants bradykinin ( BK ) and 5-hydroxytryptamine ( 5-HT ) , in addition to the influence of the calcium ionophore A23187 , on the source of AA release and 5-lipoxygenation in human neutrophils ( PMNs ) in vitro .
	manualset3
241180	10	421975	7	NULL	NULL	0	NULL	5-lipoxygenation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present studies were designed to investigate the effect of the physiological stimulants bradykinin ( BK ) and 5-hydroxytryptamine ( 5-HT ) , in addition to the influence of the calcium ionophore A23187 , on the source of AA release and 5-lipoxygenation in human neutrophils ( PMNs ) in vitro .
	manualset3
241181	11	421975	7	NULL	NULL	0	NULL	human neutrophils	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The present studies were designed to investigate the effect of the physiological stimulants bradykinin ( BK ) and 5-hydroxytryptamine ( 5-HT ) , in addition to the influence of the calcium ionophore A23187 , on the source of AA release and 5-lipoxygenation in human neutrophils ( PMNs ) in vitro .
	manualset3
241182	12	421975	7	NULL	NULL	0	NULL	PMNs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The present studies were designed to investigate the effect of the physiological stimulants bradykinin ( BK ) and 5-hydroxytryptamine ( 5-HT ) , in addition to the influence of the calcium ionophore A23187 , on the source of AA release and 5-lipoxygenation in human neutrophils ( PMNs ) in vitro .
	manualset3
241183	1	421976	7	NULL	NULL	0	NULL	single i.v. dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A single i.v. dose ( 0.1 mmol Be2 + / kg ) of beryllium chloride prolonged the duration of pentobarbital-induced sleep and zoxazolamine-induced paralysis , in rats .
	manualset3
241184	2	421976	7	NULL	NULL	0	NULL	 0.1 mmol Be2 + / kg	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A single i.v. dose ( 0.1 mmol Be2 + / kg ) of beryllium chloride prolonged the duration of pentobarbital-induced sleep and zoxazolamine-induced paralysis , in rats .
	manualset3
241185	3	421976	7	NULL	NULL	0	NULL	beryllium chloride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A single i.v. dose ( 0.1 mmol Be2 + / kg ) of beryllium chloride prolonged the duration of pentobarbital-induced sleep and zoxazolamine-induced paralysis , in rats .
	manualset3
241186	4	421976	7	NULL	NULL	0	NULL	 duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A single i.v. dose ( 0.1 mmol Be2 + / kg ) of beryllium chloride prolonged the duration of pentobarbital-induced sleep and zoxazolamine-induced paralysis , in rats .
	manualset3
241187	5	421976	7	NULL	NULL	0	NULL	pentobarbital-induced sleep	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A single i.v. dose ( 0.1 mmol Be2 + / kg ) of beryllium chloride prolonged the duration of pentobarbital-induced sleep and zoxazolamine-induced paralysis , in rats .
	manualset3
241188	6	421976	7	NULL	NULL	0	NULL	zoxazolamine-induced paralysis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A single i.v. dose ( 0.1 mmol Be2 + / kg ) of beryllium chloride prolonged the duration of pentobarbital-induced sleep and zoxazolamine-induced paralysis , in rats .
	manualset3
241189	7	421976	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	A single i.v. dose ( 0.1 mmol Be2 + / kg ) of beryllium chloride prolonged the duration of pentobarbital-induced sleep and zoxazolamine-induced paralysis , in rats .
	manualset3
241190	1	421977	7	NULL	NULL	0	NULL	Design	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Design , synthesis , and biological evaluation of new cyclic melanotropin peptide analogs selective for the human melanocortin-4 receptor .
	manualset3
241191	2	421977	7	NULL	NULL	0	NULL	synthesis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Design , synthesis , and biological evaluation of new cyclic melanotropin peptide analogs selective for the human melanocortin-4 receptor .
	manualset3
241192	3	421977	7	NULL	NULL	0	NULL	biological evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Design , synthesis , and biological evaluation of new cyclic melanotropin peptide analogs selective for the human melanocortin-4 receptor .
	manualset3
241193	4	421977	7	NULL	NULL	0	NULL	new cyclic melanotropin peptide analogs	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Design , synthesis , and biological evaluation of new cyclic melanotropin peptide analogs selective for the human melanocortin-4 receptor .
	manualset3
241194	5	421977	7	NULL	NULL	0	NULL	human melanocortin-4 receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Design , synthesis , and biological evaluation of new cyclic melanotropin peptide analogs selective for the human melanocortin-4 receptor .
	manualset3
241195	1	421978	7	NULL	NULL	0	NULL	Action	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Action of norethandrolone on disorders of calcium excretion in children .
	manualset3
241196	2	421978	7	NULL	NULL	0	NULL	norethandrolone	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Action of norethandrolone on disorders of calcium excretion in children .
	manualset3
241197	3	421978	7	NULL	NULL	0	NULL	disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Action of norethandrolone on disorders of calcium excretion in children .
	manualset3
241198	4	421978	7	NULL	NULL	0	NULL	calcium excretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Action of norethandrolone on disorders of calcium excretion in children .
	manualset3
241199	5	421978	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Action of norethandrolone on disorders of calcium excretion in children .
	manualset3
241200	2	421979	7	NULL	NULL	NULL	NULL	 recommendation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Writing letters of recommendation : where should you start ?
	manualset3
241201	1	421979	7	NULL	NULL	0	NULL	 letters	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Writing letters of recommendation : where should you start ?
	manualset3
241202	1	421980	7	NULL	NULL	0	NULL	endoscopic microsurgical technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An endoscopic microsurgical technique has been developed on the basis of the development of a new technique for hemostasis ( endocoagulation ) , which needs neither ligation nor high-frequency current , and a specific pelviscopic instrument setup for surgical therapeutic pelviscopy has been created .
	manualset3
241203	2	421980	7	NULL	NULL	0	NULL	basis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An endoscopic microsurgical technique has been developed on the basis of the development of a new technique for hemostasis ( endocoagulation ) , which needs neither ligation nor high-frequency current , and a specific pelviscopic instrument setup for surgical therapeutic pelviscopy has been created .
	manualset3
241204	3	421980	7	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An endoscopic microsurgical technique has been developed on the basis of the development of a new technique for hemostasis ( endocoagulation ) , which needs neither ligation nor high-frequency current , and a specific pelviscopic instrument setup for surgical therapeutic pelviscopy has been created .
	manualset3
241205	4	421980	7	NULL	NULL	0	NULL	new technique	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An endoscopic microsurgical technique has been developed on the basis of the development of a new technique for hemostasis ( endocoagulation ) , which needs neither ligation nor high-frequency current , and a specific pelviscopic instrument setup for surgical therapeutic pelviscopy has been created .
	manualset3
241206	5	421980	7	NULL	NULL	0	NULL	hemostasis ( endocoagulation )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An endoscopic microsurgical technique has been developed on the basis of the development of a new technique for hemostasis ( endocoagulation ) , which needs neither ligation nor high-frequency current , and a specific pelviscopic instrument setup for surgical therapeutic pelviscopy has been created .
	manualset3
241207	6	421980	7	NULL	NULL	0	NULL	ligation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An endoscopic microsurgical technique has been developed on the basis of the development of a new technique for hemostasis ( endocoagulation ) , which needs neither ligation nor high-frequency current , and a specific pelviscopic instrument setup for surgical therapeutic pelviscopy has been created .
	manualset3
241208	7	421980	7	NULL	NULL	0	NULL	high-frequency current 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	An endoscopic microsurgical technique has been developed on the basis of the development of a new technique for hemostasis ( endocoagulation ) , which needs neither ligation nor high-frequency current , and a specific pelviscopic instrument setup for surgical therapeutic pelviscopy has been created .
	manualset3
241209	8	421980	7	NULL	NULL	0	NULL	pelviscopic instrument setup	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	An endoscopic microsurgical technique has been developed on the basis of the development of a new technique for hemostasis ( endocoagulation ) , which needs neither ligation nor high-frequency current , and a specific pelviscopic instrument setup for surgical therapeutic pelviscopy has been created .
	manualset3
241210	9	421980	7	NULL	NULL	0	NULL	surgical therapeutic pelviscopy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An endoscopic microsurgical technique has been developed on the basis of the development of a new technique for hemostasis ( endocoagulation ) , which needs neither ligation nor high-frequency current , and a specific pelviscopic instrument setup for surgical therapeutic pelviscopy has been created .
	manualset3
241418	1	421981	7	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the most obvious aims in the critical postoperative period after heart surgery in children is protection of the cardiorespiratory system against stress reactions .
	manualset3
241420	2	421981	7	NULL	NULL	0	NULL	critical postoperative period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the most obvious aims in the critical postoperative period after heart surgery in children is protection of the cardiorespiratory system against stress reactions .
	manualset3
241421	3	421981	7	NULL	NULL	0	NULL	heart surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the most obvious aims in the critical postoperative period after heart surgery in children is protection of the cardiorespiratory system against stress reactions .
	manualset3
241423	4	421981	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the most obvious aims in the critical postoperative period after heart surgery in children is protection of the cardiorespiratory system against stress reactions .
	manualset3
241427	5	421981	7	NULL	NULL	0	NULL	 protection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the most obvious aims in the critical postoperative period after heart surgery in children is protection of the cardiorespiratory system against stress reactions .
	manualset3
241429	6	421981	7	NULL	NULL	0	NULL	cardiorespiratory system 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the most obvious aims in the critical postoperative period after heart surgery in children is protection of the cardiorespiratory system against stress reactions .
	manualset3
241430	7	421981	7	NULL	NULL	0	NULL	stress reactions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the most obvious aims in the critical postoperative period after heart surgery in children is protection of the cardiorespiratory system against stress reactions .
	manualset3
241440	1	421982	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the use of a roller and an air-resistance simulator can be used for ergometry and training .
	manualset3
241442	2	421982	7	NULL	NULL	0	NULL	 roller	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the use of a roller and an air-resistance simulator can be used for ergometry and training .
	manualset3
241444	3	421982	7	NULL	NULL	0	NULL	air-resistance simulator	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the use of a roller and an air-resistance simulator can be used for ergometry and training .
	manualset3
241447	4	421982	7	NULL	NULL	0	NULL	ergometry	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the use of a roller and an air-resistance simulator can be used for ergometry and training .
	manualset3
241448	5	421982	7	NULL	NULL	0	NULL	training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It is concluded that the use of a roller and an air-resistance simulator can be used for ergometry and training .
	manualset3
241454	1	421983	7	NULL	NULL	0	NULL	Coronary angiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Coronary angiography revealed a coronary artery fistula ( CAF ) and a non-significant stenosis of the left anterior descending coronary artery ( LAD ) .
	manualset3
241456	2	421983	7	NULL	NULL	NULL	NULL	coronary artery fistula ( CAF )	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coronary angiography revealed a coronary artery fistula ( CAF ) and a non-significant stenosis of the left anterior descending coronary artery ( LAD ) .
	manualset3
241457	3	421983	7	NULL	NULL	NULL	NULL	non-significant stenosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coronary angiography revealed a coronary artery fistula ( CAF ) and a non-significant stenosis of the left anterior descending coronary artery ( LAD ) .
	manualset3
241459	4	421983	7	NULL	NULL	0	NULL	left anterior descending coronary artery ( LAD )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Coronary angiography revealed a coronary artery fistula ( CAF ) and a non-significant stenosis of the left anterior descending coronary artery ( LAD ) .
	manualset3
241462	1	421984	7	NULL	NULL	0	NULL	Belt nonwearer overrepresentation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Belt nonwearer overrepresentation was found to increase with increasing levels of belt wearing in the driver population from a factor of between 2 and 5 ( depending on crash severity ) at b = 0.5 to between 5 and 10 as b approached 0.9 .
	manualset3
241464	2	421984	7	NULL	NULL	0	NULL	 increasing levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Belt nonwearer overrepresentation was found to increase with increasing levels of belt wearing in the driver population from a factor of between 2 and 5 ( depending on crash severity ) at b = 0.5 to between 5 and 10 as b approached 0.9 .
	manualset3
241465	3	421984	7	NULL	NULL	0	NULL	driver population 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Belt nonwearer overrepresentation was found to increase with increasing levels of belt wearing in the driver population from a factor of between 2 and 5 ( depending on crash severity ) at b = 0.5 to between 5 and 10 as b approached 0.9 .
	manualset3
241466	4	421984	7	NULL	NULL	0	NULL	factor	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Belt nonwearer overrepresentation was found to increase with increasing levels of belt wearing in the driver population from a factor of between 2 and 5 ( depending on crash severity ) at b = 0.5 to between 5 and 10 as b approached 0.9 .
	manualset3
241467	5	421984	7	NULL	NULL	0	NULL	2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Belt nonwearer overrepresentation was found to increase with increasing levels of belt wearing in the driver population from a factor of between 2 and 5 ( depending on crash severity ) at b = 0.5 to between 5 and 10 as b approached 0.9 .
	manualset3
241468	6	421984	7	NULL	NULL	0	NULL	5	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Belt nonwearer overrepresentation was found to increase with increasing levels of belt wearing in the driver population from a factor of between 2 and 5 ( depending on crash severity ) at b = 0.5 to between 5 and 10 as b approached 0.9 .
	manualset3
241469	7	421984	7	NULL	NULL	0	NULL	crash severity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Belt nonwearer overrepresentation was found to increase with increasing levels of belt wearing in the driver population from a factor of between 2 and 5 ( depending on crash severity ) at b = 0.5 to between 5 and 10 as b approached 0.9 .
	manualset3
241470	8	421984	7	NULL	NULL	0	NULL	b = 0.5	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Belt nonwearer overrepresentation was found to increase with increasing levels of belt wearing in the driver population from a factor of between 2 and 5 ( depending on crash severity ) at b = 0.5 to between 5 and 10 as b approached 0.9 .
	manualset3
241472	9	421984	7	NULL	NULL	0	NULL	5	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Belt nonwearer overrepresentation was found to increase with increasing levels of belt wearing in the driver population from a factor of between 2 and 5 ( depending on crash severity ) at b = 0.5 to between 5 and 10 as b approached 0.9 .
	manualset3
241473	10	421984	7	NULL	NULL	0	NULL	10	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Belt nonwearer overrepresentation was found to increase with increasing levels of belt wearing in the driver population from a factor of between 2 and 5 ( depending on crash severity ) at b = 0.5 to between 5 and 10 as b approached 0.9 .
	manualset3
241474	11	421984	7	NULL	NULL	0	NULL	b	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Belt nonwearer overrepresentation was found to increase with increasing levels of belt wearing in the driver population from a factor of between 2 and 5 ( depending on crash severity ) at b = 0.5 to between 5 and 10 as b approached 0.9 .
	manualset3
241475	12	421984	7	NULL	NULL	0	NULL	0.9	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Belt nonwearer overrepresentation was found to increase with increasing levels of belt wearing in the driver population from a factor of between 2 and 5 ( depending on crash severity ) at b = 0.5 to between 5 and 10 as b approached 0.9 .
	manualset3
241476	1	421985	7	NULL	NULL	0	NULL	 lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These lesions can range from a simple inflammatory reaction to almost complete bladder retraction .
	manualset3
241477	2	421985	7	NULL	NULL	0	NULL	simple inflammatory reaction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These lesions can range from a simple inflammatory reaction to almost complete bladder retraction .
	manualset3
241478	3	421985	7	NULL	NULL	0	NULL	complete bladder retraction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These lesions can range from a simple inflammatory reaction to almost complete bladder retraction .
	manualset3
241571	1	421986	7	NULL	NULL	0	NULL	Subacute hypoxia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Subacute hypoxia decreases voltage-activated potassium channel expression and function in pulmonary artery myocytes .
	manualset3
241573	2	421986	7	NULL	NULL	0	NULL	voltage-activated potassium channel expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subacute hypoxia decreases voltage-activated potassium channel expression and function in pulmonary artery myocytes .
	manualset3
241574	3	421986	7	NULL	NULL	0	NULL	pulmonary artery myocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Subacute hypoxia decreases voltage-activated potassium channel expression and function in pulmonary artery myocytes .
	manualset3
241577	1	421987	7	NULL	NULL	0	NULL	administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The administration of bovine growth hormone and/or 3 , 5 , 3 ' - triiodo-L-thyronine to hypophysectomized rats decreased the Ca2 + release times by different degrees and thyroid hormone was more effective than growth hormone .
	manualset3
241578	2	421987	7	NULL	NULL	0	NULL	bovine growth hormone	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The administration of bovine growth hormone and/or 3 , 5 , 3 ' - triiodo-L-thyronine to hypophysectomized rats decreased the Ca2 + release times by different degrees and thyroid hormone was more effective than growth hormone .
	manualset3
241579	3	421987	7	NULL	NULL	0	NULL	3 , 5 , 3 ' - triiodo-L-thyronine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The administration of bovine growth hormone and/or 3 , 5 , 3 ' - triiodo-L-thyronine to hypophysectomized rats decreased the Ca2 + release times by different degrees and thyroid hormone was more effective than growth hormone .
	manualset3
241580	4	421987	7	NULL	NULL	0	NULL	hypophysectomized rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The administration of bovine growth hormone and/or 3 , 5 , 3 ' - triiodo-L-thyronine to hypophysectomized rats decreased the Ca2 + release times by different degrees and thyroid hormone was more effective than growth hormone .
	manualset3
241581	5	421987	7	NULL	NULL	NULL	NULL	Ca2 + release times	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The administration of bovine growth hormone and/or 3 , 5 , 3 ' - triiodo-L-thyronine to hypophysectomized rats decreased the Ca2 + release times by different degrees and thyroid hormone was more effective than growth hormone .
	manualset3
241582	6	421987	7	NULL	NULL	0	NULL	different degrees	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The administration of bovine growth hormone and/or 3 , 5 , 3 ' - triiodo-L-thyronine to hypophysectomized rats decreased the Ca2 + release times by different degrees and thyroid hormone was more effective than growth hormone .
	manualset3
241583	7	421987	7	NULL	NULL	0	NULL	thyroid hormone 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The administration of bovine growth hormone and/or 3 , 5 , 3 ' - triiodo-L-thyronine to hypophysectomized rats decreased the Ca2 + release times by different degrees and thyroid hormone was more effective than growth hormone .
	manualset3
241584	8	421987	7	NULL	NULL	0	NULL	growth hormone	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The administration of bovine growth hormone and/or 3 , 5 , 3 ' - triiodo-L-thyronine to hypophysectomized rats decreased the Ca2 + release times by different degrees and thyroid hormone was more effective than growth hormone .
	manualset3
241585	1	421988	7	NULL	NULL	NULL	NULL	10 % solution	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	A 10 % solution of sodium fluorescein was injected IV ( 14 mg/kg of body weight ) at the same time , and pupil size , intraocular pressure , and anterior chamber fluorescence were measured for 1 hour after injections .
	manualset3
241586	2	421988	7	NULL	NULL	0	NULL	sodium fluorescein	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A 10 % solution of sodium fluorescein was injected IV ( 14 mg/kg of body weight ) at the same time , and pupil size , intraocular pressure , and anterior chamber fluorescence were measured for 1 hour after injections .
	manualset3
241587	3	421988	7	NULL	NULL	0	NULL	IV ( 14 mg/kg of body weight )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A 10 % solution of sodium fluorescein was injected IV ( 14 mg/kg of body weight ) at the same time , and pupil size , intraocular pressure , and anterior chamber fluorescence were measured for 1 hour after injections .
	manualset3
241588	4	421988	7	NULL	NULL	0	NULL	 time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	A 10 % solution of sodium fluorescein was injected IV ( 14 mg/kg of body weight ) at the same time , and pupil size , intraocular pressure , and anterior chamber fluorescence were measured for 1 hour after injections .
	manualset3
241590	5	421988	7	NULL	NULL	0	NULL	pupil size	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A 10 % solution of sodium fluorescein was injected IV ( 14 mg/kg of body weight ) at the same time , and pupil size , intraocular pressure , and anterior chamber fluorescence were measured for 1 hour after injections .
	manualset3
241591	6	421988	7	NULL	NULL	0	NULL	 intraocular pressure 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A 10 % solution of sodium fluorescein was injected IV ( 14 mg/kg of body weight ) at the same time , and pupil size , intraocular pressure , and anterior chamber fluorescence were measured for 1 hour after injections .
	manualset3
241592	7	421988	7	NULL	NULL	0	NULL	anterior chamber fluorescence	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	A 10 % solution of sodium fluorescein was injected IV ( 14 mg/kg of body weight ) at the same time , and pupil size , intraocular pressure , and anterior chamber fluorescence were measured for 1 hour after injections .
	manualset3
241593	8	421988	7	NULL	NULL	0	NULL	1 hour	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	A 10 % solution of sodium fluorescein was injected IV ( 14 mg/kg of body weight ) at the same time , and pupil size , intraocular pressure , and anterior chamber fluorescence were measured for 1 hour after injections .
	manualset3
241595	9	421988	7	NULL	NULL	0	NULL	injections	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A 10 % solution of sodium fluorescein was injected IV ( 14 mg/kg of body weight ) at the same time , and pupil size , intraocular pressure , and anterior chamber fluorescence were measured for 1 hour after injections .
	manualset3
241600	1	421989	7	NULL	NULL	0	NULL	neoplasms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The neoplasms are uncommon and are classified as sebaceous lymphadenoma , sebaceous adenoma , and sebaceous carcinoma .
	manualset3
241602	2	421989	7	NULL	NULL	NULL	NULL	sebaceous lymphadenoma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The neoplasms are uncommon and are classified as sebaceous lymphadenoma , sebaceous adenoma , and sebaceous carcinoma .
	manualset3
241603	3	421989	7	NULL	NULL	NULL	NULL	sebaceous adenoma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The neoplasms are uncommon and are classified as sebaceous lymphadenoma , sebaceous adenoma , and sebaceous carcinoma .
	manualset3
241604	4	421989	7	NULL	NULL	0	NULL	sebaceous carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The neoplasms are uncommon and are classified as sebaceous lymphadenoma , sebaceous adenoma , and sebaceous carcinoma .
	manualset3
241605	1	421990	7	NULL	NULL	0	NULL	Diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Diagnosis of renal tuberculosis by biopsy of ureteral vegetation ) .
	manualset3
241606	2	421990	7	NULL	NULL	0	NULL	renal tuberculosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Diagnosis of renal tuberculosis by biopsy of ureteral vegetation ) .
	manualset3
241607	3	421990	7	NULL	NULL	0	NULL	biopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Diagnosis of renal tuberculosis by biopsy of ureteral vegetation ) .
	manualset3
241608	4	421990	7	NULL	NULL	0	NULL	ureteral vegetation	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Diagnosis of renal tuberculosis by biopsy of ureteral vegetation ) .
	manualset3
241609	1	421991	7	NULL	NULL	0	NULL	enhanced green fluorescent protein ( EGFP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	An enhanced green fluorescent protein ( EGFP ) plasmid-based excision assay further confirmed the efficiency of the bifunctional CPP-PBase fusion protein .
	manualset3
241610	2	421991	7	NULL	NULL	0	NULL	plasmid-based excision assay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An enhanced green fluorescent protein ( EGFP ) plasmid-based excision assay further confirmed the efficiency of the bifunctional CPP-PBase fusion protein .
	manualset3
241612	3	421991	7	NULL	NULL	0	NULL	efficiency	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An enhanced green fluorescent protein ( EGFP ) plasmid-based excision assay further confirmed the efficiency of the bifunctional CPP-PBase fusion protein .
	manualset3
241615	4	421991	7	NULL	NULL	0	NULL	bifunctional CPP-PBase fusion protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	An enhanced green fluorescent protein ( EGFP ) plasmid-based excision assay further confirmed the efficiency of the bifunctional CPP-PBase fusion protein .
	manualset3
241618	1	421992	7	NULL	NULL	0	NULL	Secretion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Secretion of soluble functional insulin receptors by transfected NIH3T3 cells .
	manualset3
241619	2	421992	7	NULL	NULL	NULL	NULL	 soluble functional insulin receptors	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Secretion of soluble functional insulin receptors by transfected NIH3T3 cells .
	manualset3
241620	3	421992	7	NULL	NULL	0	NULL	transfected NIH3T3 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Secretion of soluble functional insulin receptors by transfected NIH3T3 cells .
	manualset3
241621	1	421993	7	NULL	NULL	0	NULL	X-ray microscopy ( XRM )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray microscopy ( XRM ) is the only microscopy technique that can provide high-resolution ( 30 nm ) imaging of biological specimens without the need to fix , stain or section them .
	manualset3
241622	2	421993	7	NULL	NULL	0	NULL	 microscopy technique 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray microscopy ( XRM ) is the only microscopy technique that can provide high-resolution ( 30 nm ) imaging of biological specimens without the need to fix , stain or section them .
	manualset3
241623	3	421993	7	NULL	NULL	0	NULL	high-resolution ( 30 nm ) imaging	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray microscopy ( XRM ) is the only microscopy technique that can provide high-resolution ( 30 nm ) imaging of biological specimens without the need to fix , stain or section them .
	manualset3
241624	4	421993	7	NULL	NULL	0	NULL	biological specimens	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	X-ray microscopy ( XRM ) is the only microscopy technique that can provide high-resolution ( 30 nm ) imaging of biological specimens without the need to fix , stain or section them .
	manualset3
241626	1	421994	7	NULL	NULL	0	NULL	Proteinuria	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteinuria after conversion to sirolimus in renal transplant recipients .
	manualset3
241628	2	421994	7	NULL	NULL	0	NULL	conversion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteinuria after conversion to sirolimus in renal transplant recipients .
	manualset3
241631	3	421994	7	NULL	NULL	0	NULL	sirolimus	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteinuria after conversion to sirolimus in renal transplant recipients .
	manualset3
241632	4	421994	7	NULL	NULL	0	NULL	renal transplant recipients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Proteinuria after conversion to sirolimus in renal transplant recipients .
	manualset3
241633	1	421995	7	NULL	NULL	0	NULL	Bound auxin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Bound auxin from pea stems was fractionated into water-soluble , water-insoluble/NaOH-hydrolyzable , and insoluble components .
	manualset3
241636	2	421995	7	NULL	NULL	0	NULL	pea stems 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Bound auxin from pea stems was fractionated into water-soluble , water-insoluble/NaOH-hydrolyzable , and insoluble components .
	manualset3
241638	3	421995	7	NULL	NULL	0	NULL	 water-soluble components	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Bound auxin from pea stems was fractionated into water-soluble , water-insoluble/NaOH-hydrolyzable , and insoluble components .
	manualset3
241639	4	421995	7	NULL	NULL	0	NULL	water-insoluble/NaOH-hydrolyzable components	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Bound auxin from pea stems was fractionated into water-soluble , water-insoluble/NaOH-hydrolyzable , and insoluble components .
	manualset3
241640	5	421995	7	NULL	NULL	0	NULL	insoluble components	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Bound auxin from pea stems was fractionated into water-soluble , water-insoluble/NaOH-hydrolyzable , and insoluble components .
	manualset3
241646	1	421996	7	NULL	NULL	0	NULL	enolase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	An enolase has been purified to apparent homogeneity , as measured by gel electrophoresis , some 400-fold from spinach ( Spinacia oleracea ) .
	manualset3
241647	2	421996	7	NULL	NULL	0	NULL	homogeneity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An enolase has been purified to apparent homogeneity , as measured by gel electrophoresis , some 400-fold from spinach ( Spinacia oleracea ) .
	manualset3
241648	3	421996	7	NULL	NULL	0	NULL	gel electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An enolase has been purified to apparent homogeneity , as measured by gel electrophoresis , some 400-fold from spinach ( Spinacia oleracea ) .
	manualset3
241649	4	421996	7	NULL	NULL	0	NULL	400-fold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An enolase has been purified to apparent homogeneity , as measured by gel electrophoresis , some 400-fold from spinach ( Spinacia oleracea ) .
	manualset3
241650	5	421996	7	NULL	NULL	0	NULL	spinach ( Spinacia oleracea )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	An enolase has been purified to apparent homogeneity , as measured by gel electrophoresis , some 400-fold from spinach ( Spinacia oleracea ) .
	manualset3
241688	1	421997	7	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	During the differentiation of the clonally distributed lymphocytes of mouse and man into mature resting B and T cells , their DNA becomes tightly packed into dense heterochromatin masses and exhibits very little transcriptional activity ; it also becomes extensively nicked , containing some 3000-4000 single-strand breaks per diploid genome .
	manualset3
241690	2	421997	7	NULL	NULL	0	NULL	clonally distributed lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	During the differentiation of the clonally distributed lymphocytes of mouse and man into mature resting B and T cells , their DNA becomes tightly packed into dense heterochromatin masses and exhibits very little transcriptional activity ; it also becomes extensively nicked , containing some 3000-4000 single-strand breaks per diploid genome .
	manualset3
241693	3	421997	7	NULL	NULL	0	NULL	mouse 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	During the differentiation of the clonally distributed lymphocytes of mouse and man into mature resting B and T cells , their DNA becomes tightly packed into dense heterochromatin masses and exhibits very little transcriptional activity ; it also becomes extensively nicked , containing some 3000-4000 single-strand breaks per diploid genome .
	manualset3
241694	4	421997	7	NULL	NULL	0	NULL	man	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	During the differentiation of the clonally distributed lymphocytes of mouse and man into mature resting B and T cells , their DNA becomes tightly packed into dense heterochromatin masses and exhibits very little transcriptional activity ; it also becomes extensively nicked , containing some 3000-4000 single-strand breaks per diploid genome .
	manualset3
241696	5	421997	7	NULL	NULL	0	NULL	mature resting B cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	During the differentiation of the clonally distributed lymphocytes of mouse and man into mature resting B and T cells , their DNA becomes tightly packed into dense heterochromatin masses and exhibits very little transcriptional activity ; it also becomes extensively nicked , containing some 3000-4000 single-strand breaks per diploid genome .
	manualset3
241698	6	421997	7	NULL	NULL	0	NULL	T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	During the differentiation of the clonally distributed lymphocytes of mouse and man into mature resting B and T cells , their DNA becomes tightly packed into dense heterochromatin masses and exhibits very little transcriptional activity ; it also becomes extensively nicked , containing some 3000-4000 single-strand breaks per diploid genome .
	manualset3
241701	7	421997	7	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	During the differentiation of the clonally distributed lymphocytes of mouse and man into mature resting B and T cells , their DNA becomes tightly packed into dense heterochromatin masses and exhibits very little transcriptional activity ; it also becomes extensively nicked , containing some 3000-4000 single-strand breaks per diploid genome .
	manualset3
241704	8	421997	7	NULL	NULL	0	NULL	dense heterochromatin masses 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	During the differentiation of the clonally distributed lymphocytes of mouse and man into mature resting B and T cells , their DNA becomes tightly packed into dense heterochromatin masses and exhibits very little transcriptional activity ; it also becomes extensively nicked , containing some 3000-4000 single-strand breaks per diploid genome .
	manualset3
241706	9	421997	7	NULL	NULL	0	NULL	 transcriptional activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	During the differentiation of the clonally distributed lymphocytes of mouse and man into mature resting B and T cells , their DNA becomes tightly packed into dense heterochromatin masses and exhibits very little transcriptional activity ; it also becomes extensively nicked , containing some 3000-4000 single-strand breaks per diploid genome .
	manualset3
241707	10	421997	7	NULL	NULL	NULL	NULL	3000-4000 single-strand breaks 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the differentiation of the clonally distributed lymphocytes of mouse and man into mature resting B and T cells , their DNA becomes tightly packed into dense heterochromatin masses and exhibits very little transcriptional activity ; it also becomes extensively nicked , containing some 3000-4000 single-strand breaks per diploid genome .
	manualset3
247400	11	421997	7	NULL	NULL	0	NULL	 diploid genome	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	During the differentiation of the clonally distributed lymphocytes of mouse and man into mature resting B and T cells , their DNA becomes tightly packed into dense heterochromatin masses and exhibits very little transcriptional activity ; it also becomes extensively nicked , containing some 3000-4000 single-strand breaks per diploid genome .
	manualset3
241712	1	421998	7	NULL	NULL	0	NULL	State of water	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( State of water in living tissues ( results of NMR-spin echo studies ) ) .
	manualset3
241714	2	421998	7	NULL	NULL	0	NULL	living tissues 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	( State of water in living tissues ( results of NMR-spin echo studies ) ) .
	manualset3
241715	3	421998	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( State of water in living tissues ( results of NMR-spin echo studies ) ) .
	manualset3
241717	4	421998	7	NULL	NULL	0	NULL	NMR-spin echo studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( State of water in living tissues ( results of NMR-spin echo studies ) ) .
	manualset3
241721	1	421999	7	NULL	NULL	0	NULL	 Factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Factors affecting the metabolism and distribution of phenazepam in subcellular fractions of animal hepatocytes ) .
	manualset3
241722	2	421999	7	NULL	NULL	0	NULL	metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Factors affecting the metabolism and distribution of phenazepam in subcellular fractions of animal hepatocytes ) .
	manualset3
241723	3	421999	7	NULL	NULL	0	NULL	distribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Factors affecting the metabolism and distribution of phenazepam in subcellular fractions of animal hepatocytes ) .
	manualset3
241724	4	421999	7	NULL	NULL	0	NULL	phenazepam	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Factors affecting the metabolism and distribution of phenazepam in subcellular fractions of animal hepatocytes ) .
	manualset3
241726	5	421999	7	NULL	NULL	0	NULL	subcellular fractions	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	( Factors affecting the metabolism and distribution of phenazepam in subcellular fractions of animal hepatocytes ) .
	manualset3
241727	6	421999	7	NULL	NULL	0	NULL	animal hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	( Factors affecting the metabolism and distribution of phenazepam in subcellular fractions of animal hepatocytes ) .
	manualset3
241733	1	422000	7	NULL	NULL	0	NULL	Samples	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples were then incubated in a 60 degrees C water bath for 20 min , cooled in a room temperature water bath for 40 min , then diluted with deionized , distilled water ( DDW ; 3 ml ) and again vortex-mixed .
	manualset3
241734	2	422000	7	NULL	NULL	0	NULL	60 degrees C 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples were then incubated in a 60 degrees C water bath for 20 min , cooled in a room temperature water bath for 40 min , then diluted with deionized , distilled water ( DDW ; 3 ml ) and again vortex-mixed .
	manualset3
241735	3	422000	7	NULL	NULL	0	NULL	water bath	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples were then incubated in a 60 degrees C water bath for 20 min , cooled in a room temperature water bath for 40 min , then diluted with deionized , distilled water ( DDW ; 3 ml ) and again vortex-mixed .
	manualset3
241737	4	422000	7	NULL	NULL	0	NULL	 20 min 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples were then incubated in a 60 degrees C water bath for 20 min , cooled in a room temperature water bath for 40 min , then diluted with deionized , distilled water ( DDW ; 3 ml ) and again vortex-mixed .
	manualset3
241739	5	422000	7	NULL	NULL	0	NULL	room temperature	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples were then incubated in a 60 degrees C water bath for 20 min , cooled in a room temperature water bath for 40 min , then diluted with deionized , distilled water ( DDW ; 3 ml ) and again vortex-mixed .
	manualset3
241742	6	422000	7	NULL	NULL	0	NULL	water bath 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples were then incubated in a 60 degrees C water bath for 20 min , cooled in a room temperature water bath for 40 min , then diluted with deionized , distilled water ( DDW ; 3 ml ) and again vortex-mixed .
	manualset3
241744	7	422000	7	NULL	NULL	0	NULL	 40 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples were then incubated in a 60 degrees C water bath for 20 min , cooled in a room temperature water bath for 40 min , then diluted with deionized , distilled water ( DDW ; 3 ml ) and again vortex-mixed .
	manualset3
241745	8	422000	7	NULL	NULL	0	NULL	 distilled water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples were then incubated in a 60 degrees C water bath for 20 min , cooled in a room temperature water bath for 40 min , then diluted with deionized , distilled water ( DDW ; 3 ml ) and again vortex-mixed .
	manualset3
241746	9	422000	7	NULL	NULL	0	NULL	DDW 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples were then incubated in a 60 degrees C water bath for 20 min , cooled in a room temperature water bath for 40 min , then diluted with deionized , distilled water ( DDW ; 3 ml ) and again vortex-mixed .
	manualset3
241748	10	422000	7	NULL	NULL	0	NULL	3 ml	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Samples were then incubated in a 60 degrees C water bath for 20 min , cooled in a room temperature water bath for 40 min , then diluted with deionized , distilled water ( DDW ; 3 ml ) and again vortex-mixed .
	manualset3
241749	1	422001	7	NULL	NULL	0	NULL	Stimulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of only central or only peripheral zone of the RF in nearly equal number of cases increased or decreased the sensitivity index in comparison with full cruciform figure .
	manualset3
241761	2	422001	7	NULL	NULL	0	NULL	central zone	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of only central or only peripheral zone of the RF in nearly equal number of cases increased or decreased the sensitivity index in comparison with full cruciform figure .
	manualset3
241762	3	422001	7	NULL	NULL	0	NULL	peripheral zone	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of only central or only peripheral zone of the RF in nearly equal number of cases increased or decreased the sensitivity index in comparison with full cruciform figure .
	manualset3
241763	4	422001	7	NULL	NULL	0	NULL	RF	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of only central or only peripheral zone of the RF in nearly equal number of cases increased or decreased the sensitivity index in comparison with full cruciform figure .
	manualset3
241765	5	422001	7	NULL	NULL	0	NULL	equal number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of only central or only peripheral zone of the RF in nearly equal number of cases increased or decreased the sensitivity index in comparison with full cruciform figure .
	manualset3
241767	6	422001	7	NULL	NULL	0	NULL	cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of only central or only peripheral zone of the RF in nearly equal number of cases increased or decreased the sensitivity index in comparison with full cruciform figure .
	manualset3
241775	7	422001	7	NULL	NULL	0	NULL	sensitivity index 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of only central or only peripheral zone of the RF in nearly equal number of cases increased or decreased the sensitivity index in comparison with full cruciform figure .
	manualset3
241778	8	422001	7	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulation of only central or only peripheral zone of the RF in nearly equal number of cases increased or decreased the sensitivity index in comparison with full cruciform figure .
	manualset3
241789	9	422001	7	NULL	NULL	NULL	NULL	full cruciform figure	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Stimulation of only central or only peripheral zone of the RF in nearly equal number of cases increased or decreased the sensitivity index in comparison with full cruciform figure .
	manualset3
242593	1	422002	7	NULL	NULL	0	NULL	result	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An entirely different result emerged when acrosome reactions were induced with A23187 : M42 was no longer able to prevent the AR .
	manualset3
242594	2	422002	7	NULL	NULL	0	NULL	acrosome reactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An entirely different result emerged when acrosome reactions were induced with A23187 : M42 was no longer able to prevent the AR .
	manualset3
242595	3	422002	7	NULL	NULL	0	NULL	A23187 : M42 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	An entirely different result emerged when acrosome reactions were induced with A23187 : M42 was no longer able to prevent the AR .
	manualset3
242596	4	422002	7	NULL	NULL	0	NULL	AR	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An entirely different result emerged when acrosome reactions were induced with A23187 : M42 was no longer able to prevent the AR .
	manualset3
242597	1	422003	7	NULL	NULL	0	NULL	Aceruloplasminemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Aceruloplasminemia is a disorder of iron metabolism caused by mutations in the ceruloplasmin gene .
	manualset3
242598	2	422003	7	NULL	NULL	0	NULL	disorder 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Aceruloplasminemia is a disorder of iron metabolism caused by mutations in the ceruloplasmin gene .
	manualset3
242599	3	422003	7	NULL	NULL	NULL	NULL	iron metabolism	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Aceruloplasminemia is a disorder of iron metabolism caused by mutations in the ceruloplasmin gene .
	manualset3
242600	4	422003	7	NULL	NULL	0	NULL	 mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Aceruloplasminemia is a disorder of iron metabolism caused by mutations in the ceruloplasmin gene .
	manualset3
242601	5	422003	7	NULL	NULL	0	NULL	ceruloplasmin gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Aceruloplasminemia is a disorder of iron metabolism caused by mutations in the ceruloplasmin gene .
	manualset3
242602	1	422004	7	NULL	NULL	0	NULL	dilemma	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The dilemma of delirium : clinical and research controversies regarding diagnosis and evaluation of delirium in hospitalized elderly medical patients .
	manualset3
242608	2	422004	7	NULL	NULL	0	NULL	delirium	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The dilemma of delirium : clinical and research controversies regarding diagnosis and evaluation of delirium in hospitalized elderly medical patients .
	manualset3
242609	3	422004	7	NULL	NULL	0	NULL	clinical controversies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The dilemma of delirium : clinical and research controversies regarding diagnosis and evaluation of delirium in hospitalized elderly medical patients .
	manualset3
242610	4	422004	7	NULL	NULL	0	NULL	research controversies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The dilemma of delirium : clinical and research controversies regarding diagnosis and evaluation of delirium in hospitalized elderly medical patients .
	manualset3
242613	5	422004	7	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The dilemma of delirium : clinical and research controversies regarding diagnosis and evaluation of delirium in hospitalized elderly medical patients .
	manualset3
242615	6	422004	7	NULL	NULL	0	NULL	evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The dilemma of delirium : clinical and research controversies regarding diagnosis and evaluation of delirium in hospitalized elderly medical patients .
	manualset3
242616	7	422004	7	NULL	NULL	0	NULL	delirium	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The dilemma of delirium : clinical and research controversies regarding diagnosis and evaluation of delirium in hospitalized elderly medical patients .
	manualset3
242617	8	422004	7	NULL	NULL	0	NULL	hospitalized elderly medical patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The dilemma of delirium : clinical and research controversies regarding diagnosis and evaluation of delirium in hospitalized elderly medical patients .
	manualset3
242624	1	422005	7	NULL	NULL	0	NULL	Atrial natriuretic peptide ( ANP )	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Atrial natriuretic peptide ( ANP ) has been reported to be locally synthesized in the ovary although its physiological roles are still unknown .
	manualset3
242625	2	422005	7	NULL	NULL	0	NULL	ovary	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Atrial natriuretic peptide ( ANP ) has been reported to be locally synthesized in the ovary although its physiological roles are still unknown .
	manualset3
242626	3	422005	7	NULL	NULL	0	NULL	physiological roles	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Atrial natriuretic peptide ( ANP ) has been reported to be locally synthesized in the ovary although its physiological roles are still unknown .
	manualset3
242627	1	422006	7	NULL	NULL	0	NULL	Ipsilateral shoulder pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ipsilateral shoulder pain after thoracic surgery is a distressing problem and is associated with impairment of respiratory and shoulder function .
	manualset3
242628	2	422006	7	NULL	NULL	0	NULL	thoracic surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ipsilateral shoulder pain after thoracic surgery is a distressing problem and is associated with impairment of respiratory and shoulder function .
	manualset3
242629	3	422006	7	NULL	NULL	0	NULL	distressing problem 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ipsilateral shoulder pain after thoracic surgery is a distressing problem and is associated with impairment of respiratory and shoulder function .
	manualset3
242630	4	422006	7	NULL	NULL	0	NULL	impairment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ipsilateral shoulder pain after thoracic surgery is a distressing problem and is associated with impairment of respiratory and shoulder function .
	manualset3
242631	5	422006	7	NULL	NULL	0	NULL	respiratory function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ipsilateral shoulder pain after thoracic surgery is a distressing problem and is associated with impairment of respiratory and shoulder function .
	manualset3
242632	6	422006	7	NULL	NULL	0	NULL	shoulder function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ipsilateral shoulder pain after thoracic surgery is a distressing problem and is associated with impairment of respiratory and shoulder function .
	manualset3
242633	1	422007	7	NULL	NULL	0	NULL	Ferrimagnetic particles	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Ferrimagnetic particles in the lung .
	manualset3
242634	2	422007	7	NULL	NULL	0	NULL	 lung	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ferrimagnetic particles in the lung .
	manualset3
242635	1	422008	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	It may also spare the patient from small-stomach syndrome .
	manualset3
242636	2	422008	7	NULL	NULL	0	NULL	small-stomach syndrome 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It may also spare the patient from small-stomach syndrome .
	manualset3
242637	1	422009	7	NULL	NULL	NULL	NULL	local release	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This would mainly be due to local release of activated thrombin .
	manualset3
242638	2	422009	7	NULL	NULL	0	NULL	activated thrombin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This would mainly be due to local release of activated thrombin .
	manualset3
242639	1	422010	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were divided into three groups : normal weight ( 89-120 % ideal weight ) , mildly obese ( 120-135 % ideal weight ) , and markedly obese ( 135 % ideal weight ) .
	manualset3
242640	2	422010	7	NULL	NULL	0	NULL	three groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were divided into three groups : normal weight ( 89-120 % ideal weight ) , mildly obese ( 120-135 % ideal weight ) , and markedly obese ( 135 % ideal weight ) .
	manualset3
242641	3	422010	7	NULL	NULL	NULL	NULL	normal weight 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The patients were divided into three groups : normal weight ( 89-120 % ideal weight ) , mildly obese ( 120-135 % ideal weight ) , and markedly obese ( 135 % ideal weight ) .
	manualset3
242642	4	422010	7	NULL	NULL	0	NULL	89-120 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were divided into three groups : normal weight ( 89-120 % ideal weight ) , mildly obese ( 120-135 % ideal weight ) , and markedly obese ( 135 % ideal weight ) .
	manualset3
242643	5	422010	7	NULL	NULL	0	NULL	ideal weight	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were divided into three groups : normal weight ( 89-120 % ideal weight ) , mildly obese ( 120-135 % ideal weight ) , and markedly obese ( 135 % ideal weight ) .
	manualset3
242644	6	422010	7	NULL	NULL	0	NULL	 mildly obese 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were divided into three groups : normal weight ( 89-120 % ideal weight ) , mildly obese ( 120-135 % ideal weight ) , and markedly obese ( 135 % ideal weight ) .
	manualset3
242645	7	422010	7	NULL	NULL	0	NULL	120-135 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were divided into three groups : normal weight ( 89-120 % ideal weight ) , mildly obese ( 120-135 % ideal weight ) , and markedly obese ( 135 % ideal weight ) .
	manualset3
242646	8	422010	7	NULL	NULL	0	NULL	ideal weight	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were divided into three groups : normal weight ( 89-120 % ideal weight ) , mildly obese ( 120-135 % ideal weight ) , and markedly obese ( 135 % ideal weight ) .
	manualset3
242647	9	422010	7	NULL	NULL	0	NULL	obese 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were divided into three groups : normal weight ( 89-120 % ideal weight ) , mildly obese ( 120-135 % ideal weight ) , and markedly obese ( 135 % ideal weight ) .
	manualset3
242648	10	422010	7	NULL	NULL	0	NULL	135 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were divided into three groups : normal weight ( 89-120 % ideal weight ) , mildly obese ( 120-135 % ideal weight ) , and markedly obese ( 135 % ideal weight ) .
	manualset3
242649	11	422010	7	NULL	NULL	0	NULL	ideal weight	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were divided into three groups : normal weight ( 89-120 % ideal weight ) , mildly obese ( 120-135 % ideal weight ) , and markedly obese ( 135 % ideal weight ) .
	manualset3
242650	1	422011	7	NULL	NULL	0	NULL	A	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	A in 31 % and zinc in 88.6 % of the children .
	manualset3
242651	2	422011	7	NULL	NULL	0	NULL	31 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A in 31 % and zinc in 88.6 % of the children .
	manualset3
242652	3	422011	7	NULL	NULL	0	NULL	zinc	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	A in 31 % and zinc in 88.6 % of the children .
	manualset3
242653	4	422011	7	NULL	NULL	0	NULL	88.6 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A in 31 % and zinc in 88.6 % of the children .
	manualset3
242654	5	422011	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A in 31 % and zinc in 88.6 % of the children .
	manualset3
242655	1	422012	7	NULL	NULL	0	NULL	Supreme Court 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Supreme Court clarifies the breadth of ERISA preemption .
	manualset3
242656	2	422012	7	NULL	NULL	0	NULL	breadth	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Supreme Court clarifies the breadth of ERISA preemption .
	manualset3
242657	3	422012	7	NULL	NULL	0	NULL	ERISA preemption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Supreme Court clarifies the breadth of ERISA preemption .
	manualset3
242658	1	422013	7	NULL	NULL	0	NULL	biologically active mediators	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The biologically active mediators of antigen-specific T suppressor cells can combine with antigen on cells that are specialized to present antigen ( APC ) and render these APC incapable of presenting not only the specific antigen that the product of the T suppressor cell sees but also any other antigen in or on the APC .
	manualset3
242659	2	422013	7	NULL	NULL	0	NULL	antigen-specific T suppressor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The biologically active mediators of antigen-specific T suppressor cells can combine with antigen on cells that are specialized to present antigen ( APC ) and render these APC incapable of presenting not only the specific antigen that the product of the T suppressor cell sees but also any other antigen in or on the APC .
	manualset3
242660	3	422013	7	NULL	NULL	0	NULL	antigen	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The biologically active mediators of antigen-specific T suppressor cells can combine with antigen on cells that are specialized to present antigen ( APC ) and render these APC incapable of presenting not only the specific antigen that the product of the T suppressor cell sees but also any other antigen in or on the APC .
	manualset3
242661	4	422013	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The biologically active mediators of antigen-specific T suppressor cells can combine with antigen on cells that are specialized to present antigen ( APC ) and render these APC incapable of presenting not only the specific antigen that the product of the T suppressor cell sees but also any other antigen in or on the APC .
	manualset3
242662	5	422013	7	NULL	NULL	0	NULL	antigen	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The biologically active mediators of antigen-specific T suppressor cells can combine with antigen on cells that are specialized to present antigen ( APC ) and render these APC incapable of presenting not only the specific antigen that the product of the T suppressor cell sees but also any other antigen in or on the APC .
	manualset3
242663	6	422013	7	NULL	NULL	0	NULL	APC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The biologically active mediators of antigen-specific T suppressor cells can combine with antigen on cells that are specialized to present antigen ( APC ) and render these APC incapable of presenting not only the specific antigen that the product of the T suppressor cell sees but also any other antigen in or on the APC .
	manualset3
242664	7	422013	7	NULL	NULL	0	NULL	APC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The biologically active mediators of antigen-specific T suppressor cells can combine with antigen on cells that are specialized to present antigen ( APC ) and render these APC incapable of presenting not only the specific antigen that the product of the T suppressor cell sees but also any other antigen in or on the APC .
	manualset3
242665	8	422013	7	NULL	NULL	0	NULL	specific antigen	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The biologically active mediators of antigen-specific T suppressor cells can combine with antigen on cells that are specialized to present antigen ( APC ) and render these APC incapable of presenting not only the specific antigen that the product of the T suppressor cell sees but also any other antigen in or on the APC .
	manualset3
242666	9	422013	7	NULL	NULL	0	NULL	product 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The biologically active mediators of antigen-specific T suppressor cells can combine with antigen on cells that are specialized to present antigen ( APC ) and render these APC incapable of presenting not only the specific antigen that the product of the T suppressor cell sees but also any other antigen in or on the APC .
	manualset3
242667	10	422013	7	NULL	NULL	0	NULL	T suppressor cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The biologically active mediators of antigen-specific T suppressor cells can combine with antigen on cells that are specialized to present antigen ( APC ) and render these APC incapable of presenting not only the specific antigen that the product of the T suppressor cell sees but also any other antigen in or on the APC .
	manualset3
242668	11	422013	7	NULL	NULL	0	NULL	antigen	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The biologically active mediators of antigen-specific T suppressor cells can combine with antigen on cells that are specialized to present antigen ( APC ) and render these APC incapable of presenting not only the specific antigen that the product of the T suppressor cell sees but also any other antigen in or on the APC .
	manualset3
242669	12	422013	7	NULL	NULL	0	NULL	 APC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The biologically active mediators of antigen-specific T suppressor cells can combine with antigen on cells that are specialized to present antigen ( APC ) and render these APC incapable of presenting not only the specific antigen that the product of the T suppressor cell sees but also any other antigen in or on the APC .
	manualset3
242670	1	422014	7	NULL	NULL	0	NULL	hepatitis C virus E2-NS2 region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Processing in the hepatitis C virus E2-NS2 region : identification of p7 and two distinct E2-specific products with different C termini .
	manualset3
242671	2	422014	7	NULL	NULL	0	NULL	identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Processing in the hepatitis C virus E2-NS2 region : identification of p7 and two distinct E2-specific products with different C termini .
	manualset3
242672	3	422014	7	NULL	NULL	0	NULL	p7	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Processing in the hepatitis C virus E2-NS2 region : identification of p7 and two distinct E2-specific products with different C termini .
	manualset3
242673	4	422014	7	NULL	NULL	0	NULL	two distinct E2-specific products	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Processing in the hepatitis C virus E2-NS2 region : identification of p7 and two distinct E2-specific products with different C termini .
	manualset3
242674	5	422014	7	NULL	NULL	0	NULL	C termini	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Processing in the hepatitis C virus E2-NS2 region : identification of p7 and two distinct E2-specific products with different C termini .
	manualset3
242675	1	422015	7	NULL	NULL	0	NULL	TRH neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	TRH neurons of the hypothalamic paraventricular nucleus ( PVN ) regulate thermogenesis through the activation of the hypothalamic-pituitary-thyroid axis during cold exposure .
	manualset3
242676	2	422015	7	NULL	NULL	0	NULL	hypothalamic paraventricular nucleus ( PVN )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	TRH neurons of the hypothalamic paraventricular nucleus ( PVN ) regulate thermogenesis through the activation of the hypothalamic-pituitary-thyroid axis during cold exposure .
	manualset3
242677	3	422015	7	NULL	NULL	0	NULL	 thermogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	TRH neurons of the hypothalamic paraventricular nucleus ( PVN ) regulate thermogenesis through the activation of the hypothalamic-pituitary-thyroid axis during cold exposure .
	manualset3
242678	4	422015	7	NULL	NULL	0	NULL	activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	TRH neurons of the hypothalamic paraventricular nucleus ( PVN ) regulate thermogenesis through the activation of the hypothalamic-pituitary-thyroid axis during cold exposure .
	manualset3
242679	5	422015	7	NULL	NULL	0	NULL	hypothalamic-pituitary-thyroid axis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	TRH neurons of the hypothalamic paraventricular nucleus ( PVN ) regulate thermogenesis through the activation of the hypothalamic-pituitary-thyroid axis during cold exposure .
	manualset3
242680	6	422015	7	NULL	NULL	0	NULL	 cold exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	TRH neurons of the hypothalamic paraventricular nucleus ( PVN ) regulate thermogenesis through the activation of the hypothalamic-pituitary-thyroid axis during cold exposure .
	manualset3
242681	1	422016	7	NULL	NULL	0	NULL	epidemiologic study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An epidemiologic study of voiding and bowel habits in Korean children : a nationwide multicenter study .
	manualset3
242682	2	422016	7	NULL	NULL	0	NULL	bowel habits	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An epidemiologic study of voiding and bowel habits in Korean children : a nationwide multicenter study .
	manualset3
242683	3	422016	7	NULL	NULL	0	NULL	Korean children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	An epidemiologic study of voiding and bowel habits in Korean children : a nationwide multicenter study .
	manualset3
242684	4	422016	7	NULL	NULL	NULL	NULL	nationwide multicenter study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An epidemiologic study of voiding and bowel habits in Korean children : a nationwide multicenter study .
	manualset3
242685	1	422017	7	NULL	NULL	0	NULL	Small family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Small family with key contacts : par14 and par17 parvulin proteins , relatives of pin1 , now emerge in biomedical research .
	manualset3
242686	2	422017	7	NULL	NULL	0	NULL	key contacts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Small family with key contacts : par14 and par17 parvulin proteins , relatives of pin1 , now emerge in biomedical research .
	manualset3
242687	3	422017	7	NULL	NULL	NULL	NULL	 par14 parvulin proteins	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Small family with key contacts : par14 and par17 parvulin proteins , relatives of pin1 , now emerge in biomedical research .
	manualset3
242688	4	422017	7	NULL	NULL	0	NULL	par17 parvulin proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Small family with key contacts : par14 and par17 parvulin proteins , relatives of pin1 , now emerge in biomedical research .
	manualset3
242689	5	422017	7	NULL	NULL	0	NULL	relatives	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Small family with key contacts : par14 and par17 parvulin proteins , relatives of pin1 , now emerge in biomedical research .
	manualset3
242690	6	422017	7	NULL	NULL	0	NULL	pin1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Small family with key contacts : par14 and par17 parvulin proteins , relatives of pin1 , now emerge in biomedical research .
	manualset3
242691	7	422017	7	NULL	NULL	0	NULL	 biomedical research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Small family with key contacts : par14 and par17 parvulin proteins , relatives of pin1 , now emerge in biomedical research .
	manualset3
242692	1	422018	7	NULL	NULL	0	NULL	 genome	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also found that the genome of R. prowazekii contained a nt sequence with 68 % homology to that of the rps120 gene of R. japonica .
	manualset3
242693	2	422018	7	NULL	NULL	0	NULL	R. prowazekii 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also found that the genome of R. prowazekii contained a nt sequence with 68 % homology to that of the rps120 gene of R. japonica .
	manualset3
242694	3	422018	7	NULL	NULL	0	NULL	nt sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also found that the genome of R. prowazekii contained a nt sequence with 68 % homology to that of the rps120 gene of R. japonica .
	manualset3
242695	4	422018	7	NULL	NULL	0	NULL	68 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also found that the genome of R. prowazekii contained a nt sequence with 68 % homology to that of the rps120 gene of R. japonica .
	manualset3
242696	5	422018	7	NULL	NULL	0	NULL	homology	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also found that the genome of R. prowazekii contained a nt sequence with 68 % homology to that of the rps120 gene of R. japonica .
	manualset3
242697	6	422018	7	NULL	NULL	0	NULL	rps120 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also found that the genome of R. prowazekii contained a nt sequence with 68 % homology to that of the rps120 gene of R. japonica .
	manualset3
242698	7	422018	7	NULL	NULL	0	NULL	R. japonica	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	It was also found that the genome of R. prowazekii contained a nt sequence with 68 % homology to that of the rps120 gene of R. japonica .
	manualset3
242699	1	422019	7	NULL	NULL	0	NULL	microcirculatory parameters	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We failed to observe any significant changes in the microcirculatory parameters in patients with stage III EH .
	manualset3
242700	2	422019	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We failed to observe any significant changes in the microcirculatory parameters in patients with stage III EH .
	manualset3
242701	3	422019	7	NULL	NULL	0	NULL	stage III EH	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We failed to observe any significant changes in the microcirculatory parameters in patients with stage III EH .
	manualset3
242702	1	422020	7	NULL	NULL	0	NULL	duplication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	A duplication of the masked Ph and trisomy 13 were present as additional anomalies .
	manualset3
242703	2	422020	7	NULL	NULL	0	NULL	 masked Ph 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A duplication of the masked Ph and trisomy 13 were present as additional anomalies .
	manualset3
242704	3	422020	7	NULL	NULL	0	NULL	trisomy 13	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A duplication of the masked Ph and trisomy 13 were present as additional anomalies .
	manualset3
242705	4	422020	7	NULL	NULL	0	NULL	additional anomalies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A duplication of the masked Ph and trisomy 13 were present as additional anomalies .
	manualset3
242706	1	422021	7	NULL	NULL	0	NULL	Metabolic complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic complications of urinary diversion .
	manualset3
242707	2	422021	7	NULL	NULL	0	NULL	urinary diversion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Metabolic complications of urinary diversion .
	manualset3
242708	1	422022	7	NULL	NULL	0	NULL	Synthetic TRH 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Synthetic TRH elicited a constant , prompt increase in PRL levels .
	manualset3
242709	3	422022	7	NULL	NULL	NULL	NULL	PRL levels	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Synthetic TRH elicited a constant , prompt increase in PRL levels .
	manualset3
242710	2	422022	7	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Synthetic TRH elicited a constant , prompt increase in PRL levels .
	manualset3
242711	1	422023	7	NULL	NULL	0	NULL	week 5	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	At week 5 , significant differences ( P & lt ; 0.05 ) between treatments were found for maximum aggregation rate , TXB2 values and the TXB2/6-keto-PGF 1alpha ratio .
	manualset3
242712	2	422023	7	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	At week 5 , significant differences ( P & lt ; 0.05 ) between treatments were found for maximum aggregation rate , TXB2 values and the TXB2/6-keto-PGF 1alpha ratio .
	manualset3
242713	3	422023	7	NULL	NULL	0	NULL	P & lt ; 0.05	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	At week 5 , significant differences ( P & lt ; 0.05 ) between treatments were found for maximum aggregation rate , TXB2 values and the TXB2/6-keto-PGF 1alpha ratio .
	manualset3
242714	4	422023	7	NULL	NULL	0	NULL	treatments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	At week 5 , significant differences ( P & lt ; 0.05 ) between treatments were found for maximum aggregation rate , TXB2 values and the TXB2/6-keto-PGF 1alpha ratio .
	manualset3
242715	5	422023	7	NULL	NULL	0	NULL	maximum aggregation rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	At week 5 , significant differences ( P & lt ; 0.05 ) between treatments were found for maximum aggregation rate , TXB2 values and the TXB2/6-keto-PGF 1alpha ratio .
	manualset3
242716	6	422023	7	NULL	NULL	0	NULL	TXB2 values 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	At week 5 , significant differences ( P & lt ; 0.05 ) between treatments were found for maximum aggregation rate , TXB2 values and the TXB2/6-keto-PGF 1alpha ratio .
	manualset3
242717	7	422023	7	NULL	NULL	0	NULL	 TXB2/6-keto-PGF 1alpha ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	At week 5 , significant differences ( P & lt ; 0.05 ) between treatments were found for maximum aggregation rate , TXB2 values and the TXB2/6-keto-PGF 1alpha ratio .
	manualset3
242718	1	422024	7	NULL	NULL	0	NULL	epitope	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	An epitope on VLA-6 ( alpha6beta1 ) integrin involved in migration but not adhesion is required for extravasation of murine melanoma B16F1 cells in liver .
	manualset3
242719	2	422024	7	NULL	NULL	0	NULL	VLA-6 ( alpha6beta1 ) integrin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	An epitope on VLA-6 ( alpha6beta1 ) integrin involved in migration but not adhesion is required for extravasation of murine melanoma B16F1 cells in liver .
	manualset3
242720	3	422024	7	NULL	NULL	0	NULL	 migration 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An epitope on VLA-6 ( alpha6beta1 ) integrin involved in migration but not adhesion is required for extravasation of murine melanoma B16F1 cells in liver .
	manualset3
242721	4	422024	7	NULL	NULL	0	NULL	adhesion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An epitope on VLA-6 ( alpha6beta1 ) integrin involved in migration but not adhesion is required for extravasation of murine melanoma B16F1 cells in liver .
	manualset3
242722	5	422024	7	NULL	NULL	0	NULL	extravasation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An epitope on VLA-6 ( alpha6beta1 ) integrin involved in migration but not adhesion is required for extravasation of murine melanoma B16F1 cells in liver .
	manualset3
242723	6	422024	7	NULL	NULL	0	NULL	murine melanoma B16F1 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	An epitope on VLA-6 ( alpha6beta1 ) integrin involved in migration but not adhesion is required for extravasation of murine melanoma B16F1 cells in liver .
	manualset3
242724	7	422024	7	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An epitope on VLA-6 ( alpha6beta1 ) integrin involved in migration but not adhesion is required for extravasation of murine melanoma B16F1 cells in liver .
	manualset3
242725	1	422025	7	NULL	NULL	0	NULL	 legal differences 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there are legal differences and variations in the diagnostic criteria used to define BD among its member states , brain death is accepted as the death of an individual for all legal , ethical and scientific effects .
	manualset3
242726	2	422025	7	NULL	NULL	0	NULL	variations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there are legal differences and variations in the diagnostic criteria used to define BD among its member states , brain death is accepted as the death of an individual for all legal , ethical and scientific effects .
	manualset3
242727	3	422025	7	NULL	NULL	0	NULL	diagnostic criteria	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there are legal differences and variations in the diagnostic criteria used to define BD among its member states , brain death is accepted as the death of an individual for all legal , ethical and scientific effects .
	manualset3
242728	4	422025	7	NULL	NULL	0	NULL	BD	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there are legal differences and variations in the diagnostic criteria used to define BD among its member states , brain death is accepted as the death of an individual for all legal , ethical and scientific effects .
	manualset3
242729	5	422025	7	NULL	NULL	0	NULL	member states	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there are legal differences and variations in the diagnostic criteria used to define BD among its member states , brain death is accepted as the death of an individual for all legal , ethical and scientific effects .
	manualset3
242730	6	422025	7	NULL	NULL	0	NULL	 brain death 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there are legal differences and variations in the diagnostic criteria used to define BD among its member states , brain death is accepted as the death of an individual for all legal , ethical and scientific effects .
	manualset3
242731	7	422025	7	NULL	NULL	0	NULL	death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there are legal differences and variations in the diagnostic criteria used to define BD among its member states , brain death is accepted as the death of an individual for all legal , ethical and scientific effects .
	manualset3
242732	8	422025	7	NULL	NULL	0	NULL	individual	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there are legal differences and variations in the diagnostic criteria used to define BD among its member states , brain death is accepted as the death of an individual for all legal , ethical and scientific effects .
	manualset3
242733	9	422025	7	NULL	NULL	0	NULL	legal effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there are legal differences and variations in the diagnostic criteria used to define BD among its member states , brain death is accepted as the death of an individual for all legal , ethical and scientific effects .
	manualset3
242734	10	422025	7	NULL	NULL	0	NULL	ethical effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there are legal differences and variations in the diagnostic criteria used to define BD among its member states , brain death is accepted as the death of an individual for all legal , ethical and scientific effects .
	manualset3
242735	11	422025	7	NULL	NULL	0	NULL	scientific effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although there are legal differences and variations in the diagnostic criteria used to define BD among its member states , brain death is accepted as the death of an individual for all legal , ethical and scientific effects .
	manualset3
242736	1	422026	7	NULL	NULL	0	NULL	Histamine	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Histamine also caused increases in fractional urine flow and the fractional excretion of sodium and calcium with a concomitant decrease in urine/plasma osmolality .
	manualset3
242737	2	422026	7	NULL	NULL	0	NULL	fractional urine flow	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Histamine also caused increases in fractional urine flow and the fractional excretion of sodium and calcium with a concomitant decrease in urine/plasma osmolality .
	manualset3
242738	3	422026	7	NULL	NULL	0	NULL	fractional excretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Histamine also caused increases in fractional urine flow and the fractional excretion of sodium and calcium with a concomitant decrease in urine/plasma osmolality .
	manualset3
242739	4	422026	7	NULL	NULL	0	NULL	sodium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Histamine also caused increases in fractional urine flow and the fractional excretion of sodium and calcium with a concomitant decrease in urine/plasma osmolality .
	manualset3
242740	5	422026	7	NULL	NULL	0	NULL	calcium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Histamine also caused increases in fractional urine flow and the fractional excretion of sodium and calcium with a concomitant decrease in urine/plasma osmolality .
	manualset3
242741	6	422026	7	NULL	NULL	0	NULL	concomitant decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Histamine also caused increases in fractional urine flow and the fractional excretion of sodium and calcium with a concomitant decrease in urine/plasma osmolality .
	manualset3
242742	7	422026	7	NULL	NULL	0	NULL	urine/plasma osmolality	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Histamine also caused increases in fractional urine flow and the fractional excretion of sodium and calcium with a concomitant decrease in urine/plasma osmolality .
	manualset3
242743	1	422027	7	NULL	NULL	0	NULL	HSV-1	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	HSV-1 also grows to high titers in D2 cells but without concomitant high levels of viral DNA and RNA synthesis in the infected cells .
	manualset3
242744	2	422027	7	NULL	NULL	0	NULL	high titers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	HSV-1 also grows to high titers in D2 cells but without concomitant high levels of viral DNA and RNA synthesis in the infected cells .
	manualset3
242745	3	422027	7	NULL	NULL	0	NULL	D2 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	HSV-1 also grows to high titers in D2 cells but without concomitant high levels of viral DNA and RNA synthesis in the infected cells .
	manualset3
242746	4	422027	7	NULL	NULL	0	NULL	high levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	HSV-1 also grows to high titers in D2 cells but without concomitant high levels of viral DNA and RNA synthesis in the infected cells .
	manualset3
242747	5	422027	7	NULL	NULL	0	NULL	viral DNA synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HSV-1 also grows to high titers in D2 cells but without concomitant high levels of viral DNA and RNA synthesis in the infected cells .
	manualset3
242748	6	422027	7	NULL	NULL	0	NULL	RNA synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	HSV-1 also grows to high titers in D2 cells but without concomitant high levels of viral DNA and RNA synthesis in the infected cells .
	manualset3
242749	7	422027	7	NULL	NULL	0	NULL	infected cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	HSV-1 also grows to high titers in D2 cells but without concomitant high levels of viral DNA and RNA synthesis in the infected cells .
	manualset3
242750	1	422028	7	NULL	NULL	0	NULL	Average methylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Average methylation at the H19 DMR was 61.2 % .
	manualset3
242751	2	422028	7	NULL	NULL	0	NULL	H19 DMR	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Average methylation at the H19 DMR was 61.2 % .
	manualset3
242752	3	422028	7	NULL	NULL	0	NULL	61.2 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Average methylation at the H19 DMR was 61.2 % .
	manualset3
242753	1	422029	7	NULL	NULL	NULL	NULL	Group 3 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Group 3 : roots were obturated with gutta-percha ; Group 4 : roots were restored with gutta-percha , composite , and glass fiber post ; Group 5 : roots were obturated with Resilon ; Group 6 : Roots were restored with Resilon , composite , and glass fiber post .
	manualset3
242754	2	422029	7	NULL	NULL	0	NULL	roots	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 3 : roots were obturated with gutta-percha ; Group 4 : roots were restored with gutta-percha , composite , and glass fiber post ; Group 5 : roots were obturated with Resilon ; Group 6 : Roots were restored with Resilon , composite , and glass fiber post .
	manualset3
242755	3	422029	7	NULL	NULL	0	NULL	gutta-percha	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 3 : roots were obturated with gutta-percha ; Group 4 : roots were restored with gutta-percha , composite , and glass fiber post ; Group 5 : roots were obturated with Resilon ; Group 6 : Roots were restored with Resilon , composite , and glass fiber post .
	manualset3
242756	4	422029	7	NULL	NULL	0	NULL	Group 4 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 3 : roots were obturated with gutta-percha ; Group 4 : roots were restored with gutta-percha , composite , and glass fiber post ; Group 5 : roots were obturated with Resilon ; Group 6 : Roots were restored with Resilon , composite , and glass fiber post .
	manualset3
242757	5	422029	7	NULL	NULL	0	NULL	roots	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 3 : roots were obturated with gutta-percha ; Group 4 : roots were restored with gutta-percha , composite , and glass fiber post ; Group 5 : roots were obturated with Resilon ; Group 6 : Roots were restored with Resilon , composite , and glass fiber post .
	manualset3
242758	6	422029	7	NULL	NULL	0	NULL	gutta-percha	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 3 : roots were obturated with gutta-percha ; Group 4 : roots were restored with gutta-percha , composite , and glass fiber post ; Group 5 : roots were obturated with Resilon ; Group 6 : Roots were restored with Resilon , composite , and glass fiber post .
	manualset3
242759	7	422029	7	NULL	NULL	0	NULL	glass fiber post	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 3 : roots were obturated with gutta-percha ; Group 4 : roots were restored with gutta-percha , composite , and glass fiber post ; Group 5 : roots were obturated with Resilon ; Group 6 : Roots were restored with Resilon , composite , and glass fiber post .
	manualset3
242760	8	422029	7	NULL	NULL	0	NULL	Group 5 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 3 : roots were obturated with gutta-percha ; Group 4 : roots were restored with gutta-percha , composite , and glass fiber post ; Group 5 : roots were obturated with Resilon ; Group 6 : Roots were restored with Resilon , composite , and glass fiber post .
	manualset3
242761	9	422029	7	NULL	NULL	0	NULL	roots	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 3 : roots were obturated with gutta-percha ; Group 4 : roots were restored with gutta-percha , composite , and glass fiber post ; Group 5 : roots were obturated with Resilon ; Group 6 : Roots were restored with Resilon , composite , and glass fiber post .
	manualset3
242762	10	422029	7	NULL	NULL	0	NULL	Resilon 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 3 : roots were obturated with gutta-percha ; Group 4 : roots were restored with gutta-percha , composite , and glass fiber post ; Group 5 : roots were obturated with Resilon ; Group 6 : Roots were restored with Resilon , composite , and glass fiber post .
	manualset3
242763	11	422029	7	NULL	NULL	0	NULL	Group 6	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 3 : roots were obturated with gutta-percha ; Group 4 : roots were restored with gutta-percha , composite , and glass fiber post ; Group 5 : roots were obturated with Resilon ; Group 6 : Roots were restored with Resilon , composite , and glass fiber post .
	manualset3
242764	12	422029	7	NULL	NULL	0	NULL	Roots 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 3 : roots were obturated with gutta-percha ; Group 4 : roots were restored with gutta-percha , composite , and glass fiber post ; Group 5 : roots were obturated with Resilon ; Group 6 : Roots were restored with Resilon , composite , and glass fiber post .
	manualset3
242765	13	422029	7	NULL	NULL	0	NULL	Resilon	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 3 : roots were obturated with gutta-percha ; Group 4 : roots were restored with gutta-percha , composite , and glass fiber post ; Group 5 : roots were obturated with Resilon ; Group 6 : Roots were restored with Resilon , composite , and glass fiber post .
	manualset3
242766	14	422029	7	NULL	NULL	0	NULL	composite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 3 : roots were obturated with gutta-percha ; Group 4 : roots were restored with gutta-percha , composite , and glass fiber post ; Group 5 : roots were obturated with Resilon ; Group 6 : Roots were restored with Resilon , composite , and glass fiber post .
	manualset3
242767	15	422029	7	NULL	NULL	0	NULL	glass fiber post	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 3 : roots were obturated with gutta-percha ; Group 4 : roots were restored with gutta-percha , composite , and glass fiber post ; Group 5 : roots were obturated with Resilon ; Group 6 : Roots were restored with Resilon , composite , and glass fiber post .
	manualset3
242768	16	422029	7	NULL	NULL	0	NULL	composite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Group 3 : roots were obturated with gutta-percha ; Group 4 : roots were restored with gutta-percha , composite , and glass fiber post ; Group 5 : roots were obturated with Resilon ; Group 6 : Roots were restored with Resilon , composite , and glass fiber post .
	manualset3
242769	1	422030	7	NULL	NULL	0	NULL	Young male rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Young male rats , trained in a spatial three-choice test , showed improved task acquisition after chronic treatment with piracetam ( 250 mg kg ( -1 ) ) .
	manualset3
242770	2	422030	7	NULL	NULL	0	NULL	spatial three-choice test	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Young male rats , trained in a spatial three-choice test , showed improved task acquisition after chronic treatment with piracetam ( 250 mg kg ( -1 ) ) .
	manualset3
242771	3	422030	7	NULL	NULL	0	NULL	task acquisition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Young male rats , trained in a spatial three-choice test , showed improved task acquisition after chronic treatment with piracetam ( 250 mg kg ( -1 ) ) .
	manualset3
242772	4	422030	7	NULL	NULL	0	NULL	chronic treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Young male rats , trained in a spatial three-choice test , showed improved task acquisition after chronic treatment with piracetam ( 250 mg kg ( -1 ) ) .
	manualset3
242773	5	422030	7	NULL	NULL	0	NULL	piracetam	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Young male rats , trained in a spatial three-choice test , showed improved task acquisition after chronic treatment with piracetam ( 250 mg kg ( -1 ) ) .
	manualset3
242774	6	422030	7	NULL	NULL	0	NULL	250 mg kg ( -1 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Young male rats , trained in a spatial three-choice test , showed improved task acquisition after chronic treatment with piracetam ( 250 mg kg ( -1 ) ) .
	manualset3
242996	1	422031	7	NULL	NULL	0	NULL	substantial portion	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An equally substantial portion will likely resist , however , raising deeper issues about the importance of uniformity in judicial practice .
	manualset3
243000	2	422031	7	NULL	NULL	0	NULL	deeper issues	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An equally substantial portion will likely resist , however , raising deeper issues about the importance of uniformity in judicial practice .
	manualset3
243001	3	422031	7	NULL	NULL	0	NULL	uniformity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An equally substantial portion will likely resist , however , raising deeper issues about the importance of uniformity in judicial practice .
	manualset3
243002	4	422031	7	NULL	NULL	0	NULL	judicial practice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An equally substantial portion will likely resist , however , raising deeper issues about the importance of uniformity in judicial practice .
	manualset3
243026	1	422032	7	NULL	NULL	0	NULL	 P. vitticeps	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , similar to P. vitticeps , we observed an insertion 801 bp long between the ND5 and ND6 genes .
	manualset3
243027	2	422032	7	NULL	NULL	0	NULL	 insertion 801 bp	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , similar to P. vitticeps , we observed an insertion 801 bp long between the ND5 and ND6 genes .
	manualset3
243028	3	422032	7	NULL	NULL	0	NULL	ND5 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , similar to P. vitticeps , we observed an insertion 801 bp long between the ND5 and ND6 genes .
	manualset3
243029	4	422032	7	NULL	NULL	0	NULL	ND6 genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , similar to P. vitticeps , we observed an insertion 801 bp long between the ND5 and ND6 genes .
	manualset3
243030	1	422033	7	NULL	NULL	0	NULL	Two days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Two days of dexamethasone versus 5 days of prednisone in the treatment of acute asthma : a randomized controlled trial .
	manualset3
243031	2	422033	7	NULL	NULL	0	NULL	dexamethasone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Two days of dexamethasone versus 5 days of prednisone in the treatment of acute asthma : a randomized controlled trial .
	manualset3
243032	3	422033	7	NULL	NULL	0	NULL	 5 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Two days of dexamethasone versus 5 days of prednisone in the treatment of acute asthma : a randomized controlled trial .
	manualset3
243033	4	422033	7	NULL	NULL	0	NULL	prednisone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Two days of dexamethasone versus 5 days of prednisone in the treatment of acute asthma : a randomized controlled trial .
	manualset3
243034	5	422033	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Two days of dexamethasone versus 5 days of prednisone in the treatment of acute asthma : a randomized controlled trial .
	manualset3
243035	6	422033	7	NULL	NULL	0	NULL	acute asthma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Two days of dexamethasone versus 5 days of prednisone in the treatment of acute asthma : a randomized controlled trial .
	manualset3
243036	7	422033	7	NULL	NULL	0	NULL	randomized controlled trial	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Two days of dexamethasone versus 5 days of prednisone in the treatment of acute asthma : a randomized controlled trial .
	manualset3
243037	1	422034	7	NULL	NULL	0	NULL	Anti-Id 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-Id either detected a private Id of the immunizing mAb or displayed a partial cross-reactivity with Id of other mAb to CD4 .
	manualset3
243038	2	422034	7	NULL	NULL	0	NULL	private Id 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-Id either detected a private Id of the immunizing mAb or displayed a partial cross-reactivity with Id of other mAb to CD4 .
	manualset3
243039	3	422034	7	NULL	NULL	0	NULL	immunizing mAb	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-Id either detected a private Id of the immunizing mAb or displayed a partial cross-reactivity with Id of other mAb to CD4 .
	manualset3
243040	4	422034	7	NULL	NULL	0	NULL	partial cross-reactivity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-Id either detected a private Id of the immunizing mAb or displayed a partial cross-reactivity with Id of other mAb to CD4 .
	manualset3
243041	5	422034	7	NULL	NULL	0	NULL	Id	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-Id either detected a private Id of the immunizing mAb or displayed a partial cross-reactivity with Id of other mAb to CD4 .
	manualset3
243042	6	422034	7	NULL	NULL	0	NULL	mAb	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-Id either detected a private Id of the immunizing mAb or displayed a partial cross-reactivity with Id of other mAb to CD4 .
	manualset3
243043	7	422034	7	NULL	NULL	0	NULL	CD4	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-Id either detected a private Id of the immunizing mAb or displayed a partial cross-reactivity with Id of other mAb to CD4 .
	manualset3
243044	1	422035	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings suggest that higher D2RO is related to appearance of EPS .
	manualset3
243045	2	422035	7	NULL	NULL	0	NULL	higher D2RO 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings suggest that higher D2RO is related to appearance of EPS .
	manualset3
243046	3	422035	7	NULL	NULL	0	NULL	EPS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The findings suggest that higher D2RO is related to appearance of EPS .
	manualset3
243047	1	422036	7	NULL	NULL	0	NULL	Low dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Low dose STZ also disturbed organs other than the pancreas as in high dose STZ .
	manualset3
243048	2	422036	7	NULL	NULL	0	NULL	STZ	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Low dose STZ also disturbed organs other than the pancreas as in high dose STZ .
	manualset3
243049	3	422036	7	NULL	NULL	0	NULL	 organs 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Low dose STZ also disturbed organs other than the pancreas as in high dose STZ .
	manualset3
243050	4	422036	7	NULL	NULL	0	NULL	pancreas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Low dose STZ also disturbed organs other than the pancreas as in high dose STZ .
	manualset3
243051	5	422036	7	NULL	NULL	0	NULL	high dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Low dose STZ also disturbed organs other than the pancreas as in high dose STZ .
	manualset3
243052	6	422036	7	NULL	NULL	0	NULL	STZ	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Low dose STZ also disturbed organs other than the pancreas as in high dose STZ .
	manualset3
243053	1	422037	7	NULL	NULL	0	NULL	Surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Surgery as a discipline has perhaps been slower than other specialties to embrace evidence based principles .
	manualset3
243054	2	422037	7	NULL	NULL	0	NULL	specialties	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Surgery as a discipline has perhaps been slower than other specialties to embrace evidence based principles .
	manualset3
243055	3	422037	7	NULL	NULL	0	NULL	evidence based principles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Surgery as a discipline has perhaps been slower than other specialties to embrace evidence based principles .
	manualset3
243056	1	422038	7	NULL	NULL	0	NULL	microinjection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , microinjection of histamine into bilateral FNs narrowed stride width of footprint but did not influence wire suspension , whereas microinjection of histamine into bilateral INs increased stride length and promoted suspension .
	manualset3
243057	2	422038	7	NULL	NULL	0	NULL	histamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , microinjection of histamine into bilateral FNs narrowed stride width of footprint but did not influence wire suspension , whereas microinjection of histamine into bilateral INs increased stride length and promoted suspension .
	manualset3
243058	3	422038	7	NULL	NULL	0	NULL	bilateral FNs	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , microinjection of histamine into bilateral FNs narrowed stride width of footprint but did not influence wire suspension , whereas microinjection of histamine into bilateral INs increased stride length and promoted suspension .
	manualset3
243059	4	422038	7	NULL	NULL	0	NULL	stride width 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , microinjection of histamine into bilateral FNs narrowed stride width of footprint but did not influence wire suspension , whereas microinjection of histamine into bilateral INs increased stride length and promoted suspension .
	manualset3
243060	5	422038	7	NULL	NULL	0	NULL	footprint	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , microinjection of histamine into bilateral FNs narrowed stride width of footprint but did not influence wire suspension , whereas microinjection of histamine into bilateral INs increased stride length and promoted suspension .
	manualset3
243061	6	422038	7	NULL	NULL	0	NULL	wire suspension	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , microinjection of histamine into bilateral FNs narrowed stride width of footprint but did not influence wire suspension , whereas microinjection of histamine into bilateral INs increased stride length and promoted suspension .
	manualset3
243062	7	422038	7	NULL	NULL	0	NULL	microinjection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , microinjection of histamine into bilateral FNs narrowed stride width of footprint but did not influence wire suspension , whereas microinjection of histamine into bilateral INs increased stride length and promoted suspension .
	manualset3
243063	8	422038	7	NULL	NULL	0	NULL	histamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , microinjection of histamine into bilateral FNs narrowed stride width of footprint but did not influence wire suspension , whereas microinjection of histamine into bilateral INs increased stride length and promoted suspension .
	manualset3
243064	9	422038	7	NULL	NULL	0	NULL	bilateral INs 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , microinjection of histamine into bilateral FNs narrowed stride width of footprint but did not influence wire suspension , whereas microinjection of histamine into bilateral INs increased stride length and promoted suspension .
	manualset3
243065	10	422038	7	NULL	NULL	0	NULL	stride length	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , microinjection of histamine into bilateral FNs narrowed stride width of footprint but did not influence wire suspension , whereas microinjection of histamine into bilateral INs increased stride length and promoted suspension .
	manualset3
243066	11	422038	7	NULL	NULL	0	NULL	suspension	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , microinjection of histamine into bilateral FNs narrowed stride width of footprint but did not influence wire suspension , whereas microinjection of histamine into bilateral INs increased stride length and promoted suspension .
	manualset3
243067	1	422039	7	NULL	NULL	0	NULL	No significant association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant association was observed between maternal smoking and cord plasma IgE levels .
	manualset3
243068	2	422039	7	NULL	NULL	0	NULL	maternal smoking	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant association was observed between maternal smoking and cord plasma IgE levels .
	manualset3
243069	3	422039	7	NULL	NULL	0	NULL	cord plasma IgE levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	No significant association was observed between maternal smoking and cord plasma IgE levels .
	manualset3
243070	1	422040	7	NULL	NULL	0	NULL	Three types	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Three types of sulphide oxidation pathways were found in the interface .
	manualset3
243071	2	422040	7	NULL	NULL	0	NULL	sulphide oxidation pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Three types of sulphide oxidation pathways were found in the interface .
	manualset3
243072	3	422040	7	NULL	NULL	NULL	NULL	interface	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Three types of sulphide oxidation pathways were found in the interface .
	manualset3
243073	1	422041	7	NULL	NULL	0	NULL	governmental health care service	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The governmental health care service has little to offer them in terms of care and medicine .
	manualset3
243119	2	422041	7	NULL	NULL	0	NULL	care 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The governmental health care service has little to offer them in terms of care and medicine .
	manualset3
243120	3	422041	7	NULL	NULL	0	NULL	medicine 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The governmental health care service has little to offer them in terms of care and medicine .
	manualset3
243121	1	422042	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show the diversity and complexity of mechanisms of Aux/IAA-ARF - and auxin-regulated gene expression .
	manualset3
243122	2	422042	7	NULL	NULL	0	NULL	diversity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show the diversity and complexity of mechanisms of Aux/IAA-ARF - and auxin-regulated gene expression .
	manualset3
243123	3	422042	7	NULL	NULL	0	NULL	complexity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show the diversity and complexity of mechanisms of Aux/IAA-ARF - and auxin-regulated gene expression .
	manualset3
243124	4	422042	7	NULL	NULL	0	NULL	mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show the diversity and complexity of mechanisms of Aux/IAA-ARF - and auxin-regulated gene expression .
	manualset3
243125	5	422042	7	NULL	NULL	0	NULL	Aux/IAA-ARF -gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show the diversity and complexity of mechanisms of Aux/IAA-ARF - and auxin-regulated gene expression .
	manualset3
243126	6	422042	7	NULL	NULL	0	NULL	auxin-regulated gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results show the diversity and complexity of mechanisms of Aux/IAA-ARF - and auxin-regulated gene expression .
	manualset3
243186	1	422043	7	NULL	NULL	0	NULL	Assessment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of oxidized fatty acid levels is important for understanding their homeostatic and pathophysiological roles .
	manualset3
243187	2	422043	7	NULL	NULL	0	NULL	oxidized fatty acid levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of oxidized fatty acid levels is important for understanding their homeostatic and pathophysiological roles .
	manualset3
243188	3	422043	7	NULL	NULL	0	NULL	 understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of oxidized fatty acid levels is important for understanding their homeostatic and pathophysiological roles .
	manualset3
243189	4	422043	7	NULL	NULL	0	NULL	homeostatic roles	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of oxidized fatty acid levels is important for understanding their homeostatic and pathophysiological roles .
	manualset3
243190	5	422043	7	NULL	NULL	0	NULL	pathophysiological roles	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of oxidized fatty acid levels is important for understanding their homeostatic and pathophysiological roles .
	manualset3
243191	1	422044	7	NULL	NULL	0	NULL	 syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This syndrome is caused by ectopic expression of Agouti in multiple tissues .
	manualset3
243192	2	422044	7	NULL	NULL	0	NULL	ectopic expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This syndrome is caused by ectopic expression of Agouti in multiple tissues .
	manualset3
243193	3	422044	7	NULL	NULL	0	NULL	Agouti 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This syndrome is caused by ectopic expression of Agouti in multiple tissues .
	manualset3
243194	4	422044	7	NULL	NULL	0	NULL	multiple tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	This syndrome is caused by ectopic expression of Agouti in multiple tissues .
	manualset3
243195	1	422045	7	NULL	NULL	0	NULL	Training activities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Training activities must include a training workshop and ongoing consultation during the teacher 's first experience with classroom implementation .
	manualset3
243196	2	422045	7	NULL	NULL	0	NULL	 training workshop	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Training activities must include a training workshop and ongoing consultation during the teacher 's first experience with classroom implementation .
	manualset3
243197	3	422045	7	NULL	NULL	0	NULL	ongoing consultation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Training activities must include a training workshop and ongoing consultation during the teacher 's first experience with classroom implementation .
	manualset3
243198	4	422045	7	NULL	NULL	0	NULL	teacher 's first experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Training activities must include a training workshop and ongoing consultation during the teacher 's first experience with classroom implementation .
	manualset3
243199	5	422045	7	NULL	NULL	0	NULL	classroom implementation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Training activities must include a training workshop and ongoing consultation during the teacher 's first experience with classroom implementation .
	manualset3
243200	1	422046	7	NULL	NULL	0	NULL	24-h distribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The 24-h distribution of rapid eye movement ( REM ) sleep is known to be deeply reshaped among albino rats with neurotoxic lesions in the lateral hypothalamus ( LH ) or among rodent models of human narcolepsy-cataplexy , with selective damage of orexinergic neurones .
	manualset3
243201	2	422046	7	NULL	NULL	0	NULL	rapid eye movement ( REM ) sleep	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 24-h distribution of rapid eye movement ( REM ) sleep is known to be deeply reshaped among albino rats with neurotoxic lesions in the lateral hypothalamus ( LH ) or among rodent models of human narcolepsy-cataplexy , with selective damage of orexinergic neurones .
	manualset3
243202	3	422046	7	NULL	NULL	0	NULL	albino rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The 24-h distribution of rapid eye movement ( REM ) sleep is known to be deeply reshaped among albino rats with neurotoxic lesions in the lateral hypothalamus ( LH ) or among rodent models of human narcolepsy-cataplexy , with selective damage of orexinergic neurones .
	manualset3
243203	4	422046	7	NULL	NULL	0	NULL	neurotoxic lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The 24-h distribution of rapid eye movement ( REM ) sleep is known to be deeply reshaped among albino rats with neurotoxic lesions in the lateral hypothalamus ( LH ) or among rodent models of human narcolepsy-cataplexy , with selective damage of orexinergic neurones .
	manualset3
243204	5	422046	7	NULL	NULL	0	NULL	lateral hypothalamus ( LH ) 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The 24-h distribution of rapid eye movement ( REM ) sleep is known to be deeply reshaped among albino rats with neurotoxic lesions in the lateral hypothalamus ( LH ) or among rodent models of human narcolepsy-cataplexy , with selective damage of orexinergic neurones .
	manualset3
243205	6	422046	7	NULL	NULL	0	NULL	rodent models	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The 24-h distribution of rapid eye movement ( REM ) sleep is known to be deeply reshaped among albino rats with neurotoxic lesions in the lateral hypothalamus ( LH ) or among rodent models of human narcolepsy-cataplexy , with selective damage of orexinergic neurones .
	manualset3
243206	7	422046	7	NULL	NULL	0	NULL	human narcolepsy-cataplexy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The 24-h distribution of rapid eye movement ( REM ) sleep is known to be deeply reshaped among albino rats with neurotoxic lesions in the lateral hypothalamus ( LH ) or among rodent models of human narcolepsy-cataplexy , with selective damage of orexinergic neurones .
	manualset3
243207	8	422046	7	NULL	NULL	0	NULL	selective damage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The 24-h distribution of rapid eye movement ( REM ) sleep is known to be deeply reshaped among albino rats with neurotoxic lesions in the lateral hypothalamus ( LH ) or among rodent models of human narcolepsy-cataplexy , with selective damage of orexinergic neurones .
	manualset3
243208	9	422046	7	NULL	NULL	0	NULL	orexinergic neurones	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The 24-h distribution of rapid eye movement ( REM ) sleep is known to be deeply reshaped among albino rats with neurotoxic lesions in the lateral hypothalamus ( LH ) or among rodent models of human narcolepsy-cataplexy , with selective damage of orexinergic neurones .
	manualset3
243209	1	422047	7	NULL	NULL	0	NULL	HER2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( HER2 as a marker for guiding the choice of chemotherapy in breast cancer patients ) .
	manualset3
243210	2	422047	7	NULL	NULL	0	NULL	choice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( HER2 as a marker for guiding the choice of chemotherapy in breast cancer patients ) .
	manualset3
243211	3	422047	7	NULL	NULL	0	NULL	chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( HER2 as a marker for guiding the choice of chemotherapy in breast cancer patients ) .
	manualset3
243212	4	422047	7	NULL	NULL	0	NULL	breast cancer patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( HER2 as a marker for guiding the choice of chemotherapy in breast cancer patients ) .
	manualset3
243213	5	422047	7	NULL	NULL	0	NULL	marker	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( HER2 as a marker for guiding the choice of chemotherapy in breast cancer patients ) .
	manualset3
243214	1	422048	7	NULL	NULL	0	NULL	Intracellular recording	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular recording was used to study the effect of adenosine ( 3-100 microM ) on rat locus coeruleus ( LC ) neurons in a brain slice preparation .
	manualset3
243215	2	422048	7	NULL	NULL	0	NULL	effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular recording was used to study the effect of adenosine ( 3-100 microM ) on rat locus coeruleus ( LC ) neurons in a brain slice preparation .
	manualset3
243216	3	422048	7	NULL	NULL	0	NULL	adenosine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular recording was used to study the effect of adenosine ( 3-100 microM ) on rat locus coeruleus ( LC ) neurons in a brain slice preparation .
	manualset3
243217	4	422048	7	NULL	NULL	0	NULL	3-100 microM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular recording was used to study the effect of adenosine ( 3-100 microM ) on rat locus coeruleus ( LC ) neurons in a brain slice preparation .
	manualset3
243218	5	422048	7	NULL	NULL	0	NULL	rat locus coeruleus ( LC ) neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular recording was used to study the effect of adenosine ( 3-100 microM ) on rat locus coeruleus ( LC ) neurons in a brain slice preparation .
	manualset3
243219	6	422048	7	NULL	NULL	0	NULL	brain slice preparation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Intracellular recording was used to study the effect of adenosine ( 3-100 microM ) on rat locus coeruleus ( LC ) neurons in a brain slice preparation .
	manualset3
243220	1	422049	7	NULL	NULL	0	NULL	Darkfield electron microscopy 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Darkfield electron microscopy revealed the major species to be compact oblate spheroids 12 nm in width and extended filamentous particles of average length 35 nm by 1.5 nm .
	manualset3
243221	2	422049	7	NULL	NULL	0	NULL	major species 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Darkfield electron microscopy revealed the major species to be compact oblate spheroids 12 nm in width and extended filamentous particles of average length 35 nm by 1.5 nm .
	manualset3
243222	3	422049	7	NULL	NULL	NULL	NULL	oblate spheroids 12 nm	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Darkfield electron microscopy revealed the major species to be compact oblate spheroids 12 nm in width and extended filamentous particles of average length 35 nm by 1.5 nm .
	manualset3
243223	4	422049	7	NULL	NULL	0	NULL	 width 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Darkfield electron microscopy revealed the major species to be compact oblate spheroids 12 nm in width and extended filamentous particles of average length 35 nm by 1.5 nm .
	manualset3
243224	5	422049	7	NULL	NULL	0	NULL	extended filamentous particles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Darkfield electron microscopy revealed the major species to be compact oblate spheroids 12 nm in width and extended filamentous particles of average length 35 nm by 1.5 nm .
	manualset3
243225	6	422049	7	NULL	NULL	0	NULL	average length	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Darkfield electron microscopy revealed the major species to be compact oblate spheroids 12 nm in width and extended filamentous particles of average length 35 nm by 1.5 nm .
	manualset3
243226	7	422049	7	NULL	NULL	0	NULL	35 nm	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Darkfield electron microscopy revealed the major species to be compact oblate spheroids 12 nm in width and extended filamentous particles of average length 35 nm by 1.5 nm .
	manualset3
243227	8	422049	7	NULL	NULL	0	NULL	1.5 nm	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Darkfield electron microscopy revealed the major species to be compact oblate spheroids 12 nm in width and extended filamentous particles of average length 35 nm by 1.5 nm .
	manualset3
243228	1	422050	7	NULL	NULL	0	NULL	undesirable rise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , it is essential to use them intelligently to avoid a further undesirable rise in the cost of health .
	manualset3
243229	2	422050	7	NULL	NULL	0	NULL	cost	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	However , it is essential to use them intelligently to avoid a further undesirable rise in the cost of health .
	manualset3
243230	3	422050	7	NULL	NULL	0	NULL	health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , it is essential to use them intelligently to avoid a further undesirable rise in the cost of health .
	manualset3
243231	1	422051	7	NULL	NULL	0	NULL	limited structural variability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	However , due to their limited structural variability , DSB ends generated by restriction cleavage cover probably only part of the total spectrum of naturally occurring DSB termini .
	manualset3
243232	2	422051	7	NULL	NULL	0	NULL	DSB ends	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	However , due to their limited structural variability , DSB ends generated by restriction cleavage cover probably only part of the total spectrum of naturally occurring DSB termini .
	manualset3
243233	3	422051	7	NULL	NULL	0	NULL	restriction cleavage cover	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , due to their limited structural variability , DSB ends generated by restriction cleavage cover probably only part of the total spectrum of naturally occurring DSB termini .
	manualset3
243234	4	422051	7	NULL	NULL	0	NULL	total spectrum	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	However , due to their limited structural variability , DSB ends generated by restriction cleavage cover probably only part of the total spectrum of naturally occurring DSB termini .
	manualset3
243235	5	422051	7	NULL	NULL	0	NULL	DSB termini	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	However , due to their limited structural variability , DSB ends generated by restriction cleavage cover probably only part of the total spectrum of naturally occurring DSB termini .
	manualset3
243236	1	422052	7	NULL	NULL	NULL	NULL	Systemic application 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Systemic application of tetracycline resulted in fast resolution of symptoms in both the patient and her cat .
	manualset3
243237	2	422052	7	NULL	NULL	0	NULL	tetracycline	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Systemic application of tetracycline resulted in fast resolution of symptoms in both the patient and her cat .
	manualset3
243238	3	422052	7	NULL	NULL	0	NULL	fast resolution	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Systemic application of tetracycline resulted in fast resolution of symptoms in both the patient and her cat .
	manualset3
243239	4	422052	7	NULL	NULL	0	NULL	symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Systemic application of tetracycline resulted in fast resolution of symptoms in both the patient and her cat .
	manualset3
243240	5	422052	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Systemic application of tetracycline resulted in fast resolution of symptoms in both the patient and her cat .
	manualset3
243241	6	422052	7	NULL	NULL	0	NULL	 cat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Systemic application of tetracycline resulted in fast resolution of symptoms in both the patient and her cat .
	manualset3
243242	1	422053	7	NULL	NULL	0	NULL	drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	When drugs were administered systemically , food restriction potentiated the threshold-lowering effect of amphetamine ( 0.125 , 0.25 , and 0.5 mg/kg , i.p. ) , phencyclidine ( 1.0 , 2.0 , and 3.0 mg/kg , i.p. ) , and dizocilpine ( MK-801 ) ( 0.0125 , 0.05 , and 0.1 mg/kg , i.p. ) but not nicotine ( 0.15 , 0.3 , 0.45 mg/kg , s.c. ) .
	manualset3
243243	2	422053	7	NULL	NULL	0	NULL	food restriction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When drugs were administered systemically , food restriction potentiated the threshold-lowering effect of amphetamine ( 0.125 , 0.25 , and 0.5 mg/kg , i.p. ) , phencyclidine ( 1.0 , 2.0 , and 3.0 mg/kg , i.p. ) , and dizocilpine ( MK-801 ) ( 0.0125 , 0.05 , and 0.1 mg/kg , i.p. ) but not nicotine ( 0.15 , 0.3 , 0.45 mg/kg , s.c. ) .
	manualset3
243244	3	422053	7	NULL	NULL	0	NULL	threshold-lowering effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When drugs were administered systemically , food restriction potentiated the threshold-lowering effect of amphetamine ( 0.125 , 0.25 , and 0.5 mg/kg , i.p. ) , phencyclidine ( 1.0 , 2.0 , and 3.0 mg/kg , i.p. ) , and dizocilpine ( MK-801 ) ( 0.0125 , 0.05 , and 0.1 mg/kg , i.p. ) but not nicotine ( 0.15 , 0.3 , 0.45 mg/kg , s.c. ) .
	manualset3
243245	4	422053	7	NULL	NULL	0	NULL	amphetamine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	When drugs were administered systemically , food restriction potentiated the threshold-lowering effect of amphetamine ( 0.125 , 0.25 , and 0.5 mg/kg , i.p. ) , phencyclidine ( 1.0 , 2.0 , and 3.0 mg/kg , i.p. ) , and dizocilpine ( MK-801 ) ( 0.0125 , 0.05 , and 0.1 mg/kg , i.p. ) but not nicotine ( 0.15 , 0.3 , 0.45 mg/kg , s.c. ) .
	manualset3
243246	5	422053	7	NULL	NULL	0	NULL	 0.125 mg/kg , i.p.	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When drugs were administered systemically , food restriction potentiated the threshold-lowering effect of amphetamine ( 0.125 , 0.25 , and 0.5 mg/kg , i.p. ) , phencyclidine ( 1.0 , 2.0 , and 3.0 mg/kg , i.p. ) , and dizocilpine ( MK-801 ) ( 0.0125 , 0.05 , and 0.1 mg/kg , i.p. ) but not nicotine ( 0.15 , 0.3 , 0.45 mg/kg , s.c. ) .
	manualset3
243247	6	422053	7	NULL	NULL	0	NULL	 0.25 mg/kg , i.p.	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When drugs were administered systemically , food restriction potentiated the threshold-lowering effect of amphetamine ( 0.125 , 0.25 , and 0.5 mg/kg , i.p. ) , phencyclidine ( 1.0 , 2.0 , and 3.0 mg/kg , i.p. ) , and dizocilpine ( MK-801 ) ( 0.0125 , 0.05 , and 0.1 mg/kg , i.p. ) but not nicotine ( 0.15 , 0.3 , 0.45 mg/kg , s.c. ) .
	manualset3
243248	7	422053	7	NULL	NULL	0	NULL	0.5 mg/kg , i.p.	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When drugs were administered systemically , food restriction potentiated the threshold-lowering effect of amphetamine ( 0.125 , 0.25 , and 0.5 mg/kg , i.p. ) , phencyclidine ( 1.0 , 2.0 , and 3.0 mg/kg , i.p. ) , and dizocilpine ( MK-801 ) ( 0.0125 , 0.05 , and 0.1 mg/kg , i.p. ) but not nicotine ( 0.15 , 0.3 , 0.45 mg/kg , s.c. ) .
	manualset3
243249	8	422053	7	NULL	NULL	0	NULL	phencyclidine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	When drugs were administered systemically , food restriction potentiated the threshold-lowering effect of amphetamine ( 0.125 , 0.25 , and 0.5 mg/kg , i.p. ) , phencyclidine ( 1.0 , 2.0 , and 3.0 mg/kg , i.p. ) , and dizocilpine ( MK-801 ) ( 0.0125 , 0.05 , and 0.1 mg/kg , i.p. ) but not nicotine ( 0.15 , 0.3 , 0.45 mg/kg , s.c. ) .
	manualset3
243250	9	422053	7	NULL	NULL	0	NULL	1.0 mg/kg , i.p.	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When drugs were administered systemically , food restriction potentiated the threshold-lowering effect of amphetamine ( 0.125 , 0.25 , and 0.5 mg/kg , i.p. ) , phencyclidine ( 1.0 , 2.0 , and 3.0 mg/kg , i.p. ) , and dizocilpine ( MK-801 ) ( 0.0125 , 0.05 , and 0.1 mg/kg , i.p. ) but not nicotine ( 0.15 , 0.3 , 0.45 mg/kg , s.c. ) .
	manualset3
243251	10	422053	7	NULL	NULL	0	NULL	2.0 mg/kg , i.p. 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When drugs were administered systemically , food restriction potentiated the threshold-lowering effect of amphetamine ( 0.125 , 0.25 , and 0.5 mg/kg , i.p. ) , phencyclidine ( 1.0 , 2.0 , and 3.0 mg/kg , i.p. ) , and dizocilpine ( MK-801 ) ( 0.0125 , 0.05 , and 0.1 mg/kg , i.p. ) but not nicotine ( 0.15 , 0.3 , 0.45 mg/kg , s.c. ) .
	manualset3
243252	11	422053	7	NULL	NULL	0	NULL	 3.0 mg/kg , i.p.	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When drugs were administered systemically , food restriction potentiated the threshold-lowering effect of amphetamine ( 0.125 , 0.25 , and 0.5 mg/kg , i.p. ) , phencyclidine ( 1.0 , 2.0 , and 3.0 mg/kg , i.p. ) , and dizocilpine ( MK-801 ) ( 0.0125 , 0.05 , and 0.1 mg/kg , i.p. ) but not nicotine ( 0.15 , 0.3 , 0.45 mg/kg , s.c. ) .
	manualset3
243253	12	422053	7	NULL	NULL	0	NULL	dizocilpine ( MK-801 )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	When drugs were administered systemically , food restriction potentiated the threshold-lowering effect of amphetamine ( 0.125 , 0.25 , and 0.5 mg/kg , i.p. ) , phencyclidine ( 1.0 , 2.0 , and 3.0 mg/kg , i.p. ) , and dizocilpine ( MK-801 ) ( 0.0125 , 0.05 , and 0.1 mg/kg , i.p. ) but not nicotine ( 0.15 , 0.3 , 0.45 mg/kg , s.c. ) .
	manualset3
243254	13	422053	7	NULL	NULL	0	NULL	0.0125 mg/kg , i.p.	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When drugs were administered systemically , food restriction potentiated the threshold-lowering effect of amphetamine ( 0.125 , 0.25 , and 0.5 mg/kg , i.p. ) , phencyclidine ( 1.0 , 2.0 , and 3.0 mg/kg , i.p. ) , and dizocilpine ( MK-801 ) ( 0.0125 , 0.05 , and 0.1 mg/kg , i.p. ) but not nicotine ( 0.15 , 0.3 , 0.45 mg/kg , s.c. ) .
	manualset3
243255	14	422053	7	NULL	NULL	0	NULL	 0.05 mg/kg , i.p.	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When drugs were administered systemically , food restriction potentiated the threshold-lowering effect of amphetamine ( 0.125 , 0.25 , and 0.5 mg/kg , i.p. ) , phencyclidine ( 1.0 , 2.0 , and 3.0 mg/kg , i.p. ) , and dizocilpine ( MK-801 ) ( 0.0125 , 0.05 , and 0.1 mg/kg , i.p. ) but not nicotine ( 0.15 , 0.3 , 0.45 mg/kg , s.c. ) .
	manualset3
243256	15	422053	7	NULL	NULL	0	NULL	0.1 mg/kg , i.p.	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When drugs were administered systemically , food restriction potentiated the threshold-lowering effect of amphetamine ( 0.125 , 0.25 , and 0.5 mg/kg , i.p. ) , phencyclidine ( 1.0 , 2.0 , and 3.0 mg/kg , i.p. ) , and dizocilpine ( MK-801 ) ( 0.0125 , 0.05 , and 0.1 mg/kg , i.p. ) but not nicotine ( 0.15 , 0.3 , 0.45 mg/kg , s.c. ) .
	manualset3
243257	16	422053	7	NULL	NULL	NULL	NULL	nicotine 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When drugs were administered systemically , food restriction potentiated the threshold-lowering effect of amphetamine ( 0.125 , 0.25 , and 0.5 mg/kg , i.p. ) , phencyclidine ( 1.0 , 2.0 , and 3.0 mg/kg , i.p. ) , and dizocilpine ( MK-801 ) ( 0.0125 , 0.05 , and 0.1 mg/kg , i.p. ) but not nicotine ( 0.15 , 0.3 , 0.45 mg/kg , s.c. ) .
	manualset3
243258	17	422053	7	NULL	NULL	0	NULL	 0.15 mg/kg , s.c.	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When drugs were administered systemically , food restriction potentiated the threshold-lowering effect of amphetamine ( 0.125 , 0.25 , and 0.5 mg/kg , i.p. ) , phencyclidine ( 1.0 , 2.0 , and 3.0 mg/kg , i.p. ) , and dizocilpine ( MK-801 ) ( 0.0125 , 0.05 , and 0.1 mg/kg , i.p. ) but not nicotine ( 0.15 , 0.3 , 0.45 mg/kg , s.c. ) .
	manualset3
243259	18	422053	7	NULL	NULL	0	NULL	 0.3 mg/kg , s.c.	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When drugs were administered systemically , food restriction potentiated the threshold-lowering effect of amphetamine ( 0.125 , 0.25 , and 0.5 mg/kg , i.p. ) , phencyclidine ( 1.0 , 2.0 , and 3.0 mg/kg , i.p. ) , and dizocilpine ( MK-801 ) ( 0.0125 , 0.05 , and 0.1 mg/kg , i.p. ) but not nicotine ( 0.15 , 0.3 , 0.45 mg/kg , s.c. ) .
	manualset3
243260	19	422053	7	NULL	NULL	0	NULL	0.45 mg/kg , s.c.	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When drugs were administered systemically , food restriction potentiated the threshold-lowering effect of amphetamine ( 0.125 , 0.25 , and 0.5 mg/kg , i.p. ) , phencyclidine ( 1.0 , 2.0 , and 3.0 mg/kg , i.p. ) , and dizocilpine ( MK-801 ) ( 0.0125 , 0.05 , and 0.1 mg/kg , i.p. ) but not nicotine ( 0.15 , 0.3 , 0.45 mg/kg , s.c. ) .
	manualset3
243261	1	422054	7	NULL	NULL	0	NULL	evaluation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An evaluation in the dog of cardiac sphincter substitution by interposed colon in the presence of vagotomy and Finney pyloroplasty .
	manualset3
243262	2	422054	7	NULL	NULL	0	NULL	 dog 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	An evaluation in the dog of cardiac sphincter substitution by interposed colon in the presence of vagotomy and Finney pyloroplasty .
	manualset3
243263	3	422054	7	NULL	NULL	0	NULL	cardiac sphincter substitution	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An evaluation in the dog of cardiac sphincter substitution by interposed colon in the presence of vagotomy and Finney pyloroplasty .
	manualset3
243264	4	422054	7	NULL	NULL	0	NULL	interposed colon	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An evaluation in the dog of cardiac sphincter substitution by interposed colon in the presence of vagotomy and Finney pyloroplasty .
	manualset3
243265	5	422054	7	NULL	NULL	0	NULL	vagotomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An evaluation in the dog of cardiac sphincter substitution by interposed colon in the presence of vagotomy and Finney pyloroplasty .
	manualset3
243266	6	422054	7	NULL	NULL	0	NULL	Finney pyloroplasty	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An evaluation in the dog of cardiac sphincter substitution by interposed colon in the presence of vagotomy and Finney pyloroplasty .
	manualset3
243267	1	422055	7	NULL	NULL	0	NULL	dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	At every dose administered , amiodarone was found to significantly ameliorate the deleterious effects of global ischemia .
	manualset3
243268	2	422055	7	NULL	NULL	0	NULL	 amiodarone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	At every dose administered , amiodarone was found to significantly ameliorate the deleterious effects of global ischemia .
	manualset3
243269	3	422055	7	NULL	NULL	0	NULL	deleterious effects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	At every dose administered , amiodarone was found to significantly ameliorate the deleterious effects of global ischemia .
	manualset3
243270	4	422055	7	NULL	NULL	0	NULL	global ischemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	At every dose administered , amiodarone was found to significantly ameliorate the deleterious effects of global ischemia .
	manualset3
243271	1	422056	7	NULL	NULL	0	NULL	Antibacterial properties	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibacterial properties of SCE-2787 , a new cephem antibiotic .
	manualset3
243272	2	422056	7	NULL	NULL	0	NULL	SCE-2787	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibacterial properties of SCE-2787 , a new cephem antibiotic .
	manualset3
243273	3	422056	7	NULL	NULL	0	NULL	new cephem antibiotic 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibacterial properties of SCE-2787 , a new cephem antibiotic .
	manualset3
243274	1	422057	7	NULL	NULL	0	NULL	Subcellular localization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subcellular localization of alpha-tocopherol and its effect on RNA synthesis in perfused rabbit heart .
	manualset3
243275	2	422057	7	NULL	NULL	0	NULL	alpha-tocopherol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Subcellular localization of alpha-tocopherol and its effect on RNA synthesis in perfused rabbit heart .
	manualset3
243276	3	422057	7	NULL	NULL	0	NULL	effect 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subcellular localization of alpha-tocopherol and its effect on RNA synthesis in perfused rabbit heart .
	manualset3
243277	4	422057	7	NULL	NULL	0	NULL	RNA synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subcellular localization of alpha-tocopherol and its effect on RNA synthesis in perfused rabbit heart .
	manualset3
243278	5	422057	7	NULL	NULL	0	NULL	perfused rabbit heart	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Subcellular localization of alpha-tocopherol and its effect on RNA synthesis in perfused rabbit heart .
	manualset3
243279	1	422058	7	NULL	NULL	0	NULL	 dual-labeling flow cytometric method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a dual-labeling flow cytometric method , we determined the level of expression of the leukocyte integrins and intercellular adhesion molecule 1 ( ICAM-1 ) on monocytes and lymphocytes from HIV-1-infected and uninfected individuals .
	manualset3
243280	2	422058	7	NULL	NULL	0	NULL	 level of expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a dual-labeling flow cytometric method , we determined the level of expression of the leukocyte integrins and intercellular adhesion molecule 1 ( ICAM-1 ) on monocytes and lymphocytes from HIV-1-infected and uninfected individuals .
	manualset3
243281	3	422058	7	NULL	NULL	0	NULL	 leukocyte integrins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a dual-labeling flow cytometric method , we determined the level of expression of the leukocyte integrins and intercellular adhesion molecule 1 ( ICAM-1 ) on monocytes and lymphocytes from HIV-1-infected and uninfected individuals .
	manualset3
243282	4	422058	7	NULL	NULL	0	NULL	intercellular adhesion molecule 1 ( ICAM-1 )	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a dual-labeling flow cytometric method , we determined the level of expression of the leukocyte integrins and intercellular adhesion molecule 1 ( ICAM-1 ) on monocytes and lymphocytes from HIV-1-infected and uninfected individuals .
	manualset3
243283	5	422058	7	NULL	NULL	0	NULL	monocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a dual-labeling flow cytometric method , we determined the level of expression of the leukocyte integrins and intercellular adhesion molecule 1 ( ICAM-1 ) on monocytes and lymphocytes from HIV-1-infected and uninfected individuals .
	manualset3
243284	6	422058	7	NULL	NULL	0	NULL	lymphocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a dual-labeling flow cytometric method , we determined the level of expression of the leukocyte integrins and intercellular adhesion molecule 1 ( ICAM-1 ) on monocytes and lymphocytes from HIV-1-infected and uninfected individuals .
	manualset3
243285	7	422058	7	NULL	NULL	0	NULL	HIV-1-infected individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a dual-labeling flow cytometric method , we determined the level of expression of the leukocyte integrins and intercellular adhesion molecule 1 ( ICAM-1 ) on monocytes and lymphocytes from HIV-1-infected and uninfected individuals .
	manualset3
243286	8	422058	7	NULL	NULL	0	NULL	 uninfected individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Using a dual-labeling flow cytometric method , we determined the level of expression of the leukocyte integrins and intercellular adhesion molecule 1 ( ICAM-1 ) on monocytes and lymphocytes from HIV-1-infected and uninfected individuals .
	manualset3
243287	1	422059	7	NULL	NULL	0	NULL	Fractionated electrograms	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractionated electrograms were recorded in regions where infarct healing caused wide separation of individual myocardial fibers while distorting their orientation .
	manualset3
243288	2	422059	7	NULL	NULL	0	NULL	 regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractionated electrograms were recorded in regions where infarct healing caused wide separation of individual myocardial fibers while distorting their orientation .
	manualset3
243289	3	422059	7	NULL	NULL	0	NULL	infarct healing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractionated electrograms were recorded in regions where infarct healing caused wide separation of individual myocardial fibers while distorting their orientation .
	manualset3
243290	4	422059	7	NULL	NULL	0	NULL	wide separation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractionated electrograms were recorded in regions where infarct healing caused wide separation of individual myocardial fibers while distorting their orientation .
	manualset3
243291	5	422059	7	NULL	NULL	0	NULL	individual myocardial fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractionated electrograms were recorded in regions where infarct healing caused wide separation of individual myocardial fibers while distorting their orientation .
	manualset3
243292	6	422059	7	NULL	NULL	0	NULL	orientation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractionated electrograms were recorded in regions where infarct healing caused wide separation of individual myocardial fibers while distorting their orientation .
	manualset3
243293	1	422060	7	NULL	NULL	0	NULL	Spot sampling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Spot sampling may therefore result in inaccurate estimates of nutrient digestibility .
	manualset3
243294	2	422060	7	NULL	NULL	0	NULL	inaccurate estimates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spot sampling may therefore result in inaccurate estimates of nutrient digestibility .
	manualset3
243295	3	422060	7	NULL	NULL	0	NULL	nutrient digestibility	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Spot sampling may therefore result in inaccurate estimates of nutrient digestibility .
	manualset3
243296	1	422061	7	NULL	NULL	0	NULL	SMC cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	SMC cultures at a low cell density , either actively proliferating or arrested by serum starvation and stimulated with 10 % or 2 % fetal calf serum ( FCS ) in parallel to treatment , are subject to a 52-h treatment phase with a test compound .
	manualset3
243297	2	422061	7	NULL	NULL	0	NULL	low cell density	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	SMC cultures at a low cell density , either actively proliferating or arrested by serum starvation and stimulated with 10 % or 2 % fetal calf serum ( FCS ) in parallel to treatment , are subject to a 52-h treatment phase with a test compound .
	manualset3
243298	3	422061	7	NULL	NULL	0	NULL	serum starvation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	SMC cultures at a low cell density , either actively proliferating or arrested by serum starvation and stimulated with 10 % or 2 % fetal calf serum ( FCS ) in parallel to treatment , are subject to a 52-h treatment phase with a test compound .
	manualset3
243299	4	422061	7	NULL	NULL	0	NULL	10 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	SMC cultures at a low cell density , either actively proliferating or arrested by serum starvation and stimulated with 10 % or 2 % fetal calf serum ( FCS ) in parallel to treatment , are subject to a 52-h treatment phase with a test compound .
	manualset3
243300	5	422061	7	NULL	NULL	0	NULL	2 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	SMC cultures at a low cell density , either actively proliferating or arrested by serum starvation and stimulated with 10 % or 2 % fetal calf serum ( FCS ) in parallel to treatment , are subject to a 52-h treatment phase with a test compound .
	manualset3
243301	6	422061	7	NULL	NULL	0	NULL	fetal calf serum ( FCS )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	SMC cultures at a low cell density , either actively proliferating or arrested by serum starvation and stimulated with 10 % or 2 % fetal calf serum ( FCS ) in parallel to treatment , are subject to a 52-h treatment phase with a test compound .
	manualset3
243302	7	422061	7	NULL	NULL	NULL	NULL	 treatment	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	SMC cultures at a low cell density , either actively proliferating or arrested by serum starvation and stimulated with 10 % or 2 % fetal calf serum ( FCS ) in parallel to treatment , are subject to a 52-h treatment phase with a test compound .
	manualset3
243303	8	422061	7	NULL	NULL	0	NULL	 52-h treatment phase	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	SMC cultures at a low cell density , either actively proliferating or arrested by serum starvation and stimulated with 10 % or 2 % fetal calf serum ( FCS ) in parallel to treatment , are subject to a 52-h treatment phase with a test compound .
	manualset3
243304	9	422061	7	NULL	NULL	0	NULL	 test compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	SMC cultures at a low cell density , either actively proliferating or arrested by serum starvation and stimulated with 10 % or 2 % fetal calf serum ( FCS ) in parallel to treatment , are subject to a 52-h treatment phase with a test compound .
	manualset3
243305	1	422062	7	NULL	NULL	0	NULL	Mycobacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycobacteria , including Mycobacterium tuberculosis ( Mtb ) and Mycobacterium smegmatis , unlike most well studied prokaryotes , encode two ClpP homologs , ClpP1 and ClpP2 , in a single operon .
	manualset3
243306	2	422062	7	NULL	NULL	0	NULL	Mycobacterium tuberculosis ( Mtb )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycobacteria , including Mycobacterium tuberculosis ( Mtb ) and Mycobacterium smegmatis , unlike most well studied prokaryotes , encode two ClpP homologs , ClpP1 and ClpP2 , in a single operon .
	manualset3
243307	3	422062	7	NULL	NULL	0	NULL	Mycobacterium smegmatis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycobacteria , including Mycobacterium tuberculosis ( Mtb ) and Mycobacterium smegmatis , unlike most well studied prokaryotes , encode two ClpP homologs , ClpP1 and ClpP2 , in a single operon .
	manualset3
243308	4	422062	7	NULL	NULL	0	NULL	prokaryotes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycobacteria , including Mycobacterium tuberculosis ( Mtb ) and Mycobacterium smegmatis , unlike most well studied prokaryotes , encode two ClpP homologs , ClpP1 and ClpP2 , in a single operon .
	manualset3
243309	5	422062	7	NULL	NULL	0	NULL	two ClpP homologs	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycobacteria , including Mycobacterium tuberculosis ( Mtb ) and Mycobacterium smegmatis , unlike most well studied prokaryotes , encode two ClpP homologs , ClpP1 and ClpP2 , in a single operon .
	manualset3
243310	6	422062	7	NULL	NULL	0	NULL	ClpP1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycobacteria , including Mycobacterium tuberculosis ( Mtb ) and Mycobacterium smegmatis , unlike most well studied prokaryotes , encode two ClpP homologs , ClpP1 and ClpP2 , in a single operon .
	manualset3
243311	7	422062	7	NULL	NULL	0	NULL	ClpP2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycobacteria , including Mycobacterium tuberculosis ( Mtb ) and Mycobacterium smegmatis , unlike most well studied prokaryotes , encode two ClpP homologs , ClpP1 and ClpP2 , in a single operon .
	manualset3
243312	8	422062	7	NULL	NULL	0	NULL	single operon	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Mycobacteria , including Mycobacterium tuberculosis ( Mtb ) and Mycobacterium smegmatis , unlike most well studied prokaryotes , encode two ClpP homologs , ClpP1 and ClpP2 , in a single operon .
	manualset3
243313	1	422063	7	NULL	NULL	0	NULL	 benefits 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessing the benefits of rosiglitazone in women with polycystic ovary syndrome through its effects on insulin-like growth factor 1 , insulin-like growth factor-binding protein-3 and insulin resistance : a pilot study .
	manualset3
243314	2	422063	7	NULL	NULL	0	NULL	rosiglitazone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessing the benefits of rosiglitazone in women with polycystic ovary syndrome through its effects on insulin-like growth factor 1 , insulin-like growth factor-binding protein-3 and insulin resistance : a pilot study .
	manualset3
243315	3	422063	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessing the benefits of rosiglitazone in women with polycystic ovary syndrome through its effects on insulin-like growth factor 1 , insulin-like growth factor-binding protein-3 and insulin resistance : a pilot study .
	manualset3
243316	4	422063	7	NULL	NULL	0	NULL	polycystic ovary syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessing the benefits of rosiglitazone in women with polycystic ovary syndrome through its effects on insulin-like growth factor 1 , insulin-like growth factor-binding protein-3 and insulin resistance : a pilot study .
	manualset3
243317	5	422063	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessing the benefits of rosiglitazone in women with polycystic ovary syndrome through its effects on insulin-like growth factor 1 , insulin-like growth factor-binding protein-3 and insulin resistance : a pilot study .
	manualset3
243318	6	422063	7	NULL	NULL	0	NULL	insulin-like growth factor 1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessing the benefits of rosiglitazone in women with polycystic ovary syndrome through its effects on insulin-like growth factor 1 , insulin-like growth factor-binding protein-3 and insulin resistance : a pilot study .
	manualset3
243319	7	422063	7	NULL	NULL	0	NULL	insulin-like growth factor-binding protein-3 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessing the benefits of rosiglitazone in women with polycystic ovary syndrome through its effects on insulin-like growth factor 1 , insulin-like growth factor-binding protein-3 and insulin resistance : a pilot study .
	manualset3
243320	8	422063	7	NULL	NULL	0	NULL	insulin resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessing the benefits of rosiglitazone in women with polycystic ovary syndrome through its effects on insulin-like growth factor 1 , insulin-like growth factor-binding protein-3 and insulin resistance : a pilot study .
	manualset3
243321	9	422063	7	NULL	NULL	0	NULL	pilot study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessing the benefits of rosiglitazone in women with polycystic ovary syndrome through its effects on insulin-like growth factor 1 , insulin-like growth factor-binding protein-3 and insulin resistance : a pilot study .
	manualset3
243322	1	422064	7	NULL	NULL	NULL	NULL	increased mitochondrial specific activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The increased mitochondrial specific activity of short-chain acyl-CoA dehydrogenase during starvation may result from an increased availability of flavin coenzyme or an increase in enzyme catalytic efficiency .
	manualset3
243323	2	422064	7	NULL	NULL	0	NULL	short-chain acyl-CoA dehydrogenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased mitochondrial specific activity of short-chain acyl-CoA dehydrogenase during starvation may result from an increased availability of flavin coenzyme or an increase in enzyme catalytic efficiency .
	manualset3
243324	3	422064	7	NULL	NULL	0	NULL	starvation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased mitochondrial specific activity of short-chain acyl-CoA dehydrogenase during starvation may result from an increased availability of flavin coenzyme or an increase in enzyme catalytic efficiency .
	manualset3
243325	4	422064	7	NULL	NULL	NULL	NULL	increased availability 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The increased mitochondrial specific activity of short-chain acyl-CoA dehydrogenase during starvation may result from an increased availability of flavin coenzyme or an increase in enzyme catalytic efficiency .
	manualset3
243326	5	422064	7	NULL	NULL	0	NULL	flavin coenzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased mitochondrial specific activity of short-chain acyl-CoA dehydrogenase during starvation may result from an increased availability of flavin coenzyme or an increase in enzyme catalytic efficiency .
	manualset3
243327	6	422064	7	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased mitochondrial specific activity of short-chain acyl-CoA dehydrogenase during starvation may result from an increased availability of flavin coenzyme or an increase in enzyme catalytic efficiency .
	manualset3
243328	7	422064	7	NULL	NULL	0	NULL	enzyme catalytic efficiency	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The increased mitochondrial specific activity of short-chain acyl-CoA dehydrogenase during starvation may result from an increased availability of flavin coenzyme or an increase in enzyme catalytic efficiency .
	manualset3
243329	1	422065	7	NULL	NULL	0	NULL	conjugated polymer materials	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For conjugated polymer materials , there is currently a major gap in understanding between the fundamental properties observed in single molecule measurements and the bulk electronic properties extracted from measurements of highly heterogeneous thin films .
	manualset3
243330	2	422065	7	NULL	NULL	0	NULL	 major gap	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For conjugated polymer materials , there is currently a major gap in understanding between the fundamental properties observed in single molecule measurements and the bulk electronic properties extracted from measurements of highly heterogeneous thin films .
	manualset3
243331	3	422065	7	NULL	NULL	0	NULL	understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For conjugated polymer materials , there is currently a major gap in understanding between the fundamental properties observed in single molecule measurements and the bulk electronic properties extracted from measurements of highly heterogeneous thin films .
	manualset3
243332	4	422065	7	NULL	NULL	0	NULL	fundamental properties	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For conjugated polymer materials , there is currently a major gap in understanding between the fundamental properties observed in single molecule measurements and the bulk electronic properties extracted from measurements of highly heterogeneous thin films .
	manualset3
243333	5	422065	7	NULL	NULL	0	NULL	single molecule measurements	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For conjugated polymer materials , there is currently a major gap in understanding between the fundamental properties observed in single molecule measurements and the bulk electronic properties extracted from measurements of highly heterogeneous thin films .
	manualset3
243334	6	422065	7	NULL	NULL	0	NULL	bulk electronic properties 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For conjugated polymer materials , there is currently a major gap in understanding between the fundamental properties observed in single molecule measurements and the bulk electronic properties extracted from measurements of highly heterogeneous thin films .
	manualset3
243335	7	422065	7	NULL	NULL	0	NULL	measurements	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For conjugated polymer materials , there is currently a major gap in understanding between the fundamental properties observed in single molecule measurements and the bulk electronic properties extracted from measurements of highly heterogeneous thin films .
	manualset3
243336	8	422065	7	NULL	NULL	0	NULL	highly heterogeneous thin films	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For conjugated polymer materials , there is currently a major gap in understanding between the fundamental properties observed in single molecule measurements and the bulk electronic properties extracted from measurements of highly heterogeneous thin films .
	manualset3
243337	1	422066	7	NULL	NULL	0	NULL	cornstarch preparations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Both exposed cornstarch preparations inhibited specific binding of anti-latex IgE antibodies to latex proteins in a dose-response manner .
	manualset3
243338	2	422066	7	NULL	NULL	0	NULL	specific binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Both exposed cornstarch preparations inhibited specific binding of anti-latex IgE antibodies to latex proteins in a dose-response manner .
	manualset3
243339	3	422066	7	NULL	NULL	0	NULL	anti-latex IgE antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Both exposed cornstarch preparations inhibited specific binding of anti-latex IgE antibodies to latex proteins in a dose-response manner .
	manualset3
243340	4	422066	7	NULL	NULL	0	NULL	latex proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Both exposed cornstarch preparations inhibited specific binding of anti-latex IgE antibodies to latex proteins in a dose-response manner .
	manualset3
243341	5	422066	7	NULL	NULL	0	NULL	 dose-response manner	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Both exposed cornstarch preparations inhibited specific binding of anti-latex IgE antibodies to latex proteins in a dose-response manner .
	manualset3
243342	1	422067	7	NULL	NULL	0	NULL	Feeding diets	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Feeding diets with different protein contents for 1 or 4 weeks did not influence NPY gene expression in goldfish brain .
	manualset3
243343	2	422067	7	NULL	NULL	0	NULL	different protein contents	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Feeding diets with different protein contents for 1 or 4 weeks did not influence NPY gene expression in goldfish brain .
	manualset3
243344	3	422067	7	NULL	NULL	0	NULL	1 week	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Feeding diets with different protein contents for 1 or 4 weeks did not influence NPY gene expression in goldfish brain .
	manualset3
243345	4	422067	7	NULL	NULL	0	NULL	4 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Feeding diets with different protein contents for 1 or 4 weeks did not influence NPY gene expression in goldfish brain .
	manualset3
243346	5	422067	7	NULL	NULL	0	NULL	NPY gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Feeding diets with different protein contents for 1 or 4 weeks did not influence NPY gene expression in goldfish brain .
	manualset3
243347	6	422067	7	NULL	NULL	0	NULL	goldfish brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Feeding diets with different protein contents for 1 or 4 weeks did not influence NPY gene expression in goldfish brain .
	manualset3
243570	1	422068	7	NULL	NULL	0	NULL	Genotoxic evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Genotoxic evaluation of a methanolic extract of Verbascum thapsus using micronucleus test in mouse bone marrow .
	manualset3
243571	2	422068	7	NULL	NULL	0	NULL	methanolic extract	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Genotoxic evaluation of a methanolic extract of Verbascum thapsus using micronucleus test in mouse bone marrow .
	manualset3
243572	3	422068	7	NULL	NULL	0	NULL	Verbascum thapsus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Genotoxic evaluation of a methanolic extract of Verbascum thapsus using micronucleus test in mouse bone marrow .
	manualset3
243573	4	422068	7	NULL	NULL	0	NULL	micronucleus test 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Genotoxic evaluation of a methanolic extract of Verbascum thapsus using micronucleus test in mouse bone marrow .
	manualset3
243574	5	422068	7	NULL	NULL	0	NULL	mouse bone marrow	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Genotoxic evaluation of a methanolic extract of Verbascum thapsus using micronucleus test in mouse bone marrow .
	manualset3
243603	1	422069	7	NULL	NULL	0	NULL	Diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Diagnosis of states of ketosis in pediatrics ) .
	manualset3
243604	2	422069	7	NULL	NULL	0	NULL	states	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Diagnosis of states of ketosis in pediatrics ) .
	manualset3
243605	3	422069	7	NULL	NULL	0	NULL	ketosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Diagnosis of states of ketosis in pediatrics ) .
	manualset3
243606	4	422069	7	NULL	NULL	0	NULL	pediatrics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Diagnosis of states of ketosis in pediatrics ) .
	manualset3
243607	1	422070	7	NULL	NULL	0	NULL	Empire Blue Cross and Blue Shield 's proposal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Empire Blue Cross and Blue Shield 's proposal to restructure as a for-profit company and establish an independent charitable foundation .
	manualset3
243608	2	422070	7	NULL	NULL	0	NULL	for-profit company	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Empire Blue Cross and Blue Shield 's proposal to restructure as a for-profit company and establish an independent charitable foundation .
	manualset3
243609	3	422070	7	NULL	NULL	0	NULL	independent charitable foundation	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Empire Blue Cross and Blue Shield 's proposal to restructure as a for-profit company and establish an independent charitable foundation .
	manualset3
243610	1	422071	7	NULL	NULL	0	NULL	Antibody scores	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibody scores were rather more scattered in school children .
	manualset3
243611	2	422071	7	NULL	NULL	0	NULL	school children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibody scores were rather more scattered in school children .
	manualset3
243612	1	422072	7	NULL	NULL	0	NULL	FCCP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	FCCP also efficiently induced apoptosis .
	manualset3
243613	2	422072	7	NULL	NULL	0	NULL	apoptosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	FCCP also efficiently induced apoptosis .
	manualset3
243614	1	422073	7	NULL	NULL	0	NULL	summary 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , CLL B cells express Ig transcriptional factor OCT-1 , OCT-2 , and NF-KB constitutively .
	manualset3
243615	2	422073	7	NULL	NULL	0	NULL	 CLL B cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , CLL B cells express Ig transcriptional factor OCT-1 , OCT-2 , and NF-KB constitutively .
	manualset3
243616	3	422073	7	NULL	NULL	0	NULL	Ig transcriptional factor OCT-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , CLL B cells express Ig transcriptional factor OCT-1 , OCT-2 , and NF-KB constitutively .
	manualset3
243617	4	422073	7	NULL	NULL	0	NULL	OCT-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , CLL B cells express Ig transcriptional factor OCT-1 , OCT-2 , and NF-KB constitutively .
	manualset3
243618	5	422073	7	NULL	NULL	0	NULL	NF-KB	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In summary , CLL B cells express Ig transcriptional factor OCT-1 , OCT-2 , and NF-KB constitutively .
	manualset3
243619	1	422074	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that the differences in reactivity recorded between beta 2m and IgG Fab , kappa and lambda chains , all structurally related , are quantitative rather than qualitative .
	manualset3
243620	2	422074	7	NULL	NULL	0	NULL	differences 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that the differences in reactivity recorded between beta 2m and IgG Fab , kappa and lambda chains , all structurally related , are quantitative rather than qualitative .
	manualset3
243621	3	422074	7	NULL	NULL	0	NULL	reactivity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that the differences in reactivity recorded between beta 2m and IgG Fab , kappa and lambda chains , all structurally related , are quantitative rather than qualitative .
	manualset3
243622	4	422074	7	NULL	NULL	0	NULL	beta 2m	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that the differences in reactivity recorded between beta 2m and IgG Fab , kappa and lambda chains , all structurally related , are quantitative rather than qualitative .
	manualset3
243623	5	422074	7	NULL	NULL	0	NULL	IgG Fab	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that the differences in reactivity recorded between beta 2m and IgG Fab , kappa and lambda chains , all structurally related , are quantitative rather than qualitative .
	manualset3
243624	6	422074	7	NULL	NULL	0	NULL	kappa chain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that the differences in reactivity recorded between beta 2m and IgG Fab , kappa and lambda chains , all structurally related , are quantitative rather than qualitative .
	manualset3
243625	7	422074	7	NULL	NULL	0	NULL	lambda chains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Our results indicate that the differences in reactivity recorded between beta 2m and IgG Fab , kappa and lambda chains , all structurally related , are quantitative rather than qualitative .
	manualset3
243626	1	422075	7	NULL	NULL	0	NULL	Moricizine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Moricizine is extensively ( 92 % to 95 % ) bound to plasma protein .
	manualset3
243627	2	422075	7	NULL	NULL	0	NULL	92 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moricizine is extensively ( 92 % to 95 % ) bound to plasma protein .
	manualset3
243628	3	422075	7	NULL	NULL	0	NULL	95 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Moricizine is extensively ( 92 % to 95 % ) bound to plasma protein .
	manualset3
243629	4	422075	7	NULL	NULL	0	NULL	plasma protein	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Moricizine is extensively ( 92 % to 95 % ) bound to plasma protein .
	manualset3
243630	1	422076	7	NULL	NULL	0	NULL	innate immune system 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This innate immune system thereby recognizes hypoxic injury and triggers a systemic inflammatory response through the generation of C3a and subsequent activation of the NF-kappaB system .
	manualset3
243631	2	422076	7	NULL	NULL	0	NULL	hypoxic injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This innate immune system thereby recognizes hypoxic injury and triggers a systemic inflammatory response through the generation of C3a and subsequent activation of the NF-kappaB system .
	manualset3
243632	3	422076	7	NULL	NULL	0	NULL	systemic inflammatory response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This innate immune system thereby recognizes hypoxic injury and triggers a systemic inflammatory response through the generation of C3a and subsequent activation of the NF-kappaB system .
	manualset3
243633	4	422076	7	NULL	NULL	0	NULL	generation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This innate immune system thereby recognizes hypoxic injury and triggers a systemic inflammatory response through the generation of C3a and subsequent activation of the NF-kappaB system .
	manualset3
243634	5	422076	7	NULL	NULL	0	NULL	C3a	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This innate immune system thereby recognizes hypoxic injury and triggers a systemic inflammatory response through the generation of C3a and subsequent activation of the NF-kappaB system .
	manualset3
243635	6	422076	7	NULL	NULL	0	NULL	activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This innate immune system thereby recognizes hypoxic injury and triggers a systemic inflammatory response through the generation of C3a and subsequent activation of the NF-kappaB system .
	manualset3
243636	7	422076	7	NULL	NULL	0	NULL	NF-kappaB system	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This innate immune system thereby recognizes hypoxic injury and triggers a systemic inflammatory response through the generation of C3a and subsequent activation of the NF-kappaB system .
	manualset3
243637	1	422077	7	NULL	NULL	0	NULL	TBI	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	TBI occurs as a result of motor vehicle crashes , falls , and sports-related events .
	manualset3
243638	2	422077	7	NULL	NULL	0	NULL	motor vehicle crashes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	TBI occurs as a result of motor vehicle crashes , falls , and sports-related events .
	manualset3
243639	3	422077	7	NULL	NULL	0	NULL	falls	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	TBI occurs as a result of motor vehicle crashes , falls , and sports-related events .
	manualset3
243640	4	422077	7	NULL	NULL	0	NULL	sports-related events	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	TBI occurs as a result of motor vehicle crashes , falls , and sports-related events .
	manualset3
243641	1	422078	7	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies of welders exposed to zinc fumes .
	manualset3
243642	2	422078	7	NULL	NULL	0	NULL	welders	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies of welders exposed to zinc fumes .
	manualset3
243643	3	422078	7	NULL	NULL	0	NULL	 zinc fumes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies of welders exposed to zinc fumes .
	manualset3
243644	1	422079	7	NULL	NULL	0	NULL	Previous studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies examined the in vivo distribution of PTD-containing fusion proteins following administration via different routes , including portal vein , intravenous , intraperitoneal , and oral administration .
	manualset3
243645	2	422079	7	NULL	NULL	0	NULL	in vivo distribution 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies examined the in vivo distribution of PTD-containing fusion proteins following administration via different routes , including portal vein , intravenous , intraperitoneal , and oral administration .
	manualset3
243646	3	422079	7	NULL	NULL	0	NULL	PTD-containing fusion proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies examined the in vivo distribution of PTD-containing fusion proteins following administration via different routes , including portal vein , intravenous , intraperitoneal , and oral administration .
	manualset3
243647	4	422079	7	NULL	NULL	0	NULL	administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies examined the in vivo distribution of PTD-containing fusion proteins following administration via different routes , including portal vein , intravenous , intraperitoneal , and oral administration .
	manualset3
243648	5	422079	7	NULL	NULL	0	NULL	different routes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies examined the in vivo distribution of PTD-containing fusion proteins following administration via different routes , including portal vein , intravenous , intraperitoneal , and oral administration .
	manualset3
243649	6	422079	7	NULL	NULL	0	NULL	portal vein administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies examined the in vivo distribution of PTD-containing fusion proteins following administration via different routes , including portal vein , intravenous , intraperitoneal , and oral administration .
	manualset3
243650	7	422079	7	NULL	NULL	0	NULL	 intravenous administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies examined the in vivo distribution of PTD-containing fusion proteins following administration via different routes , including portal vein , intravenous , intraperitoneal , and oral administration .
	manualset3
243651	8	422079	7	NULL	NULL	0	NULL	intraperitoneal administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies examined the in vivo distribution of PTD-containing fusion proteins following administration via different routes , including portal vein , intravenous , intraperitoneal , and oral administration .
	manualset3
243652	9	422079	7	NULL	NULL	0	NULL	oral administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Previous studies examined the in vivo distribution of PTD-containing fusion proteins following administration via different routes , including portal vein , intravenous , intraperitoneal , and oral administration .
	manualset3
243653	1	422080	7	NULL	NULL	0	NULL	spotlight 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Suddenly , the spotlight has turned on the academics who 've studied creativity for decades .
	manualset3
243654	2	422080	7	NULL	NULL	0	NULL	academics	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Suddenly , the spotlight has turned on the academics who 've studied creativity for decades .
	manualset3
243655	3	422080	7	NULL	NULL	0	NULL	decades	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Suddenly , the spotlight has turned on the academics who 've studied creativity for decades .
	manualset3
243656	1	422081	7	NULL	NULL	0	NULL	Guillain-Barr syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Guillain-Barr syndrome after vaccination with purified tetanus toxoid .
	manualset3
243657	2	422081	7	NULL	NULL	0	NULL	vaccination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Guillain-Barr syndrome after vaccination with purified tetanus toxoid .
	manualset3
243658	3	422081	7	NULL	NULL	0	NULL	purified tetanus toxoid	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Guillain-Barr syndrome after vaccination with purified tetanus toxoid .
	manualset3
243659	1	422082	7	NULL	NULL	0	NULL	 method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This method of nailing was also used in patients with plates that had previously been removed .
	manualset3
243660	2	422082	7	NULL	NULL	0	NULL	nailing 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This method of nailing was also used in patients with plates that had previously been removed .
	manualset3
243661	3	422082	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This method of nailing was also used in patients with plates that had previously been removed .
	manualset3
243662	4	422082	7	NULL	NULL	0	NULL	plates	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	This method of nailing was also used in patients with plates that had previously been removed .
	manualset3
243663	1	422083	7	NULL	NULL	0	NULL	Suramin 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Suramin and heparin inhibited DNA-dependent protein kinase activity with IC ( 50 ) of 1.7 microM and 0.27 microg ml ( -1 ) respectively .
	manualset3
243664	2	422083	7	NULL	NULL	0	NULL	heparin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Suramin and heparin inhibited DNA-dependent protein kinase activity with IC ( 50 ) of 1.7 microM and 0.27 microg ml ( -1 ) respectively .
	manualset3
243665	3	422083	7	NULL	NULL	0	NULL	DNA-dependent protein kinase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Suramin and heparin inhibited DNA-dependent protein kinase activity with IC ( 50 ) of 1.7 microM and 0.27 microg ml ( -1 ) respectively .
	manualset3
243666	4	422083	7	NULL	NULL	0	NULL	IC ( 50 ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Suramin and heparin inhibited DNA-dependent protein kinase activity with IC ( 50 ) of 1.7 microM and 0.27 microg ml ( -1 ) respectively .
	manualset3
243667	5	422083	7	NULL	NULL	0	NULL	1.7 microM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Suramin and heparin inhibited DNA-dependent protein kinase activity with IC ( 50 ) of 1.7 microM and 0.27 microg ml ( -1 ) respectively .
	manualset3
243668	6	422083	7	NULL	NULL	0	NULL	 0.27 microg ml ( -1 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Suramin and heparin inhibited DNA-dependent protein kinase activity with IC ( 50 ) of 1.7 microM and 0.27 microg ml ( -1 ) respectively .
	manualset3
243669	1	422084	7	NULL	NULL	0	NULL	 evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An evaluation of the effects of INSIGHTS on the behavior of inner city primary school children .
	manualset3
243670	2	422084	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An evaluation of the effects of INSIGHTS on the behavior of inner city primary school children .
	manualset3
243671	3	422084	7	NULL	NULL	0	NULL	INSIGHTS	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An evaluation of the effects of INSIGHTS on the behavior of inner city primary school children .
	manualset3
243672	4	422084	7	NULL	NULL	0	NULL	behavior	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An evaluation of the effects of INSIGHTS on the behavior of inner city primary school children .
	manualset3
243673	5	422084	7	NULL	NULL	0	NULL	inner city primary school children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	An evaluation of the effects of INSIGHTS on the behavior of inner city primary school children .
	manualset3
243674	1	422085	7	NULL	NULL	0	NULL	Several studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Several studies have implicated a defect in DNA mismatch repair in the pathogenesis of this disease .
	manualset3
243675	2	422085	7	NULL	NULL	0	NULL	 defect 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Several studies have implicated a defect in DNA mismatch repair in the pathogenesis of this disease .
	manualset3
243676	3	422085	7	NULL	NULL	0	NULL	DNA mismatch repair	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several studies have implicated a defect in DNA mismatch repair in the pathogenesis of this disease .
	manualset3
243677	4	422085	7	NULL	NULL	0	NULL	pathogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Several studies have implicated a defect in DNA mismatch repair in the pathogenesis of this disease .
	manualset3
243678	5	422085	7	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Several studies have implicated a defect in DNA mismatch repair in the pathogenesis of this disease .
	manualset3
243679	1	422086	7	NULL	NULL	0	NULL	Role 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Role of Omi/HtrA2 in renal tubular cells apoptosis induced by post asphyxial serum of neonate ) .
	manualset3
243680	2	422086	7	NULL	NULL	0	NULL	Omi/HtrA2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Role of Omi/HtrA2 in renal tubular cells apoptosis induced by post asphyxial serum of neonate ) .
	manualset3
243681	3	422086	7	NULL	NULL	0	NULL	renal tubular cells apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Role of Omi/HtrA2 in renal tubular cells apoptosis induced by post asphyxial serum of neonate ) .
	manualset3
243682	4	422086	7	NULL	NULL	NULL	NULL	post asphyxial serum	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Role of Omi/HtrA2 in renal tubular cells apoptosis induced by post asphyxial serum of neonate ) .
	manualset3
243683	5	422086	7	NULL	NULL	0	NULL	 neonate 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Role of Omi/HtrA2 in renal tubular cells apoptosis induced by post asphyxial serum of neonate ) .
	manualset3
243684	1	422087	7	NULL	NULL	0	NULL	reduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	There was an unexpected reduction in serum fibrinogen levels , from 288 to 253 mg/dl ( p less than 0.01 ) .
	manualset3
243685	2	422087	7	NULL	NULL	0	NULL	serum fibrinogen levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was an unexpected reduction in serum fibrinogen levels , from 288 to 253 mg/dl ( p less than 0.01 ) .
	manualset3
243686	3	422087	7	NULL	NULL	0	NULL	288 mg/dl	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was an unexpected reduction in serum fibrinogen levels , from 288 to 253 mg/dl ( p less than 0.01 ) .
	manualset3
243687	4	422087	7	NULL	NULL	0	NULL	253 mg/dl	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was an unexpected reduction in serum fibrinogen levels , from 288 to 253 mg/dl ( p less than 0.01 ) .
	manualset3
243688	5	422087	7	NULL	NULL	0	NULL	p less than 0.01	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	There was an unexpected reduction in serum fibrinogen levels , from 288 to 253 mg/dl ( p less than 0.01 ) .
	manualset3
243689	1	422088	7	NULL	NULL	0	NULL	Update	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Update : influenza activity -- United States and worldwide , and the composition of the 1991-92 influenza vaccine .
	manualset3
243690	2	422088	7	NULL	NULL	0	NULL	influenza activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Update : influenza activity -- United States and worldwide , and the composition of the 1991-92 influenza vaccine .
	manualset3
243691	3	422088	7	NULL	NULL	0	NULL	United States	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Update : influenza activity -- United States and worldwide , and the composition of the 1991-92 influenza vaccine .
	manualset3
243692	4	422088	7	NULL	NULL	0	NULL	worldwide	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Update : influenza activity -- United States and worldwide , and the composition of the 1991-92 influenza vaccine .
	manualset3
243693	5	422088	7	NULL	NULL	0	NULL	composition	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Update : influenza activity -- United States and worldwide , and the composition of the 1991-92 influenza vaccine .
	manualset3
243694	6	422088	7	NULL	NULL	0	NULL	1991-92 influenza vaccine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Update : influenza activity -- United States and worldwide , and the composition of the 1991-92 influenza vaccine .
	manualset3
243695	1	422089	7	NULL	NULL	0	NULL	experimental evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , emerging experimental evidence suggests that VEGF-targeting therapy induced less tumor cell-specific cytotoxicity , allowing residual cells to become more resistant and eventually develop a more malignant phenotype .
	manualset3
243696	2	422089	7	NULL	NULL	0	NULL	VEGF-targeting therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , emerging experimental evidence suggests that VEGF-targeting therapy induced less tumor cell-specific cytotoxicity , allowing residual cells to become more resistant and eventually develop a more malignant phenotype .
	manualset3
243697	3	422089	7	NULL	NULL	0	NULL	tumor cell-specific cytotoxicity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , emerging experimental evidence suggests that VEGF-targeting therapy induced less tumor cell-specific cytotoxicity , allowing residual cells to become more resistant and eventually develop a more malignant phenotype .
	manualset3
243698	4	422089	7	NULL	NULL	0	NULL	residual cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , emerging experimental evidence suggests that VEGF-targeting therapy induced less tumor cell-specific cytotoxicity , allowing residual cells to become more resistant and eventually develop a more malignant phenotype .
	manualset3
243699	5	422089	7	NULL	NULL	0	NULL	malignant phenotype	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Indeed , emerging experimental evidence suggests that VEGF-targeting therapy induced less tumor cell-specific cytotoxicity , allowing residual cells to become more resistant and eventually develop a more malignant phenotype .
	manualset3
243700	1	422090	7	NULL	NULL	0	NULL	 aim	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim is to train medical students for the practical use of their knowledge , utilizing patient data in a total hospital information system .
	manualset3
243701	2	422090	7	NULL	NULL	0	NULL	medical students 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim is to train medical students for the practical use of their knowledge , utilizing patient data in a total hospital information system .
	manualset3
243702	3	422090	7	NULL	NULL	0	NULL	 practical use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim is to train medical students for the practical use of their knowledge , utilizing patient data in a total hospital information system .
	manualset3
243703	4	422090	7	NULL	NULL	0	NULL	knowledge	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim is to train medical students for the practical use of their knowledge , utilizing patient data in a total hospital information system .
	manualset3
243704	5	422090	7	NULL	NULL	0	NULL	patient data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim is to train medical students for the practical use of their knowledge , utilizing patient data in a total hospital information system .
	manualset3
243705	6	422090	7	NULL	NULL	0	NULL	total hospital information system	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The aim is to train medical students for the practical use of their knowledge , utilizing patient data in a total hospital information system .
	manualset3
243706	1	422091	7	NULL	NULL	0	NULL	diseased conspirator	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( The diseased conspirator : Federico Confaloniere : an epileptic according to history and a cardiopath according to medical history ) .
	manualset3
243707	2	422091	7	NULL	NULL	0	NULL	Federico Confaloniere	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( The diseased conspirator : Federico Confaloniere : an epileptic according to history and a cardiopath according to medical history ) .
	manualset3
243708	3	422091	7	NULL	NULL	0	NULL	epileptic	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( The diseased conspirator : Federico Confaloniere : an epileptic according to history and a cardiopath according to medical history ) .
	manualset3
243709	4	422091	7	NULL	NULL	0	NULL	history	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( The diseased conspirator : Federico Confaloniere : an epileptic according to history and a cardiopath according to medical history ) .
	manualset3
243710	5	422091	7	NULL	NULL	NULL	NULL	cardiopath	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( The diseased conspirator : Federico Confaloniere : an epileptic according to history and a cardiopath according to medical history ) .
	manualset3
243711	6	422091	7	NULL	NULL	0	NULL	medical history	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( The diseased conspirator : Federico Confaloniere : an epileptic according to history and a cardiopath according to medical history ) .
	manualset3
243712	1	422092	7	NULL	NULL	0	NULL	Small increases	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Small increases in amorphous material were noted between the collagen fibrils , but the stromal lamellae were otherwise well preserved and oriented .
	manualset3
243713	2	422092	7	NULL	NULL	0	NULL	amorphous material	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Small increases in amorphous material were noted between the collagen fibrils , but the stromal lamellae were otherwise well preserved and oriented .
	manualset3
243714	3	422092	7	NULL	NULL	0	NULL	collagen fibrils	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Small increases in amorphous material were noted between the collagen fibrils , but the stromal lamellae were otherwise well preserved and oriented .
	manualset3
243715	4	422092	7	NULL	NULL	0	NULL	stromal lamellae	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Small increases in amorphous material were noted between the collagen fibrils , but the stromal lamellae were otherwise well preserved and oriented .
	manualset3
243716	1	422093	7	NULL	NULL	0	NULL	Eight patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Eight patients have been reoperated on for valve-related complications ( 1.17 % per patient-year ) : five primary deteriorations , two paravalvular leaks and one case of endocarditis .
	manualset3
243717	2	422093	7	NULL	NULL	0	NULL	valve-related complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Eight patients have been reoperated on for valve-related complications ( 1.17 % per patient-year ) : five primary deteriorations , two paravalvular leaks and one case of endocarditis .
	manualset3
243718	3	422093	7	NULL	NULL	0	NULL	1.17 % per patient-year 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Eight patients have been reoperated on for valve-related complications ( 1.17 % per patient-year ) : five primary deteriorations , two paravalvular leaks and one case of endocarditis .
	manualset3
243719	4	422093	7	NULL	NULL	0	NULL	five primary deteriorations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Eight patients have been reoperated on for valve-related complications ( 1.17 % per patient-year ) : five primary deteriorations , two paravalvular leaks and one case of endocarditis .
	manualset3
243720	5	422093	7	NULL	NULL	0	NULL	two paravalvular leaks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Eight patients have been reoperated on for valve-related complications ( 1.17 % per patient-year ) : five primary deteriorations , two paravalvular leaks and one case of endocarditis .
	manualset3
243721	6	422093	7	NULL	NULL	0	NULL	one case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Eight patients have been reoperated on for valve-related complications ( 1.17 % per patient-year ) : five primary deteriorations , two paravalvular leaks and one case of endocarditis .
	manualset3
243722	7	422093	7	NULL	NULL	0	NULL	endocarditis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Eight patients have been reoperated on for valve-related complications ( 1.17 % per patient-year ) : five primary deteriorations , two paravalvular leaks and one case of endocarditis .
	manualset3
243723	1	422094	7	NULL	NULL	0	NULL	evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An evaluation of ultrastrong polyethylene fiber as an ophthalmic suture .
	manualset3
243724	2	422094	7	NULL	NULL	0	NULL	ultrastrong polyethylene fiber	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An evaluation of ultrastrong polyethylene fiber as an ophthalmic suture .
	manualset3
243725	3	422094	7	NULL	NULL	0	NULL	ophthalmic suture	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An evaluation of ultrastrong polyethylene fiber as an ophthalmic suture .
	manualset3
243726	1	422095	7	NULL	NULL	0	NULL	snails	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The snails were infected at a juvenile stage , and release of cercariae started on Day 55 after exposure .
	manualset3
243727	2	422095	7	NULL	NULL	0	NULL	 juvenile stage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The snails were infected at a juvenile stage , and release of cercariae started on Day 55 after exposure .
	manualset3
243728	3	422095	7	NULL	NULL	0	NULL	release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The snails were infected at a juvenile stage , and release of cercariae started on Day 55 after exposure .
	manualset3
243729	4	422095	7	NULL	NULL	0	NULL	 cercariae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The snails were infected at a juvenile stage , and release of cercariae started on Day 55 after exposure .
	manualset3
243730	5	422095	7	NULL	NULL	0	NULL	Day 55	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	The snails were infected at a juvenile stage , and release of cercariae started on Day 55 after exposure .
	manualset3
243731	6	422095	7	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The snails were infected at a juvenile stage , and release of cercariae started on Day 55 after exposure .
	manualset3
243732	1	422096	7	NULL	NULL	0	NULL	ECG	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , ECG appears less sensitive than echo in the detection of LVH .
	manualset3
243733	2	422096	7	NULL	NULL	0	NULL	 echo	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , ECG appears less sensitive than echo in the detection of LVH .
	manualset3
243734	3	422096	7	NULL	NULL	0	NULL	detection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , ECG appears less sensitive than echo in the detection of LVH .
	manualset3
243735	4	422096	7	NULL	NULL	0	NULL	LVH	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Thus , ECG appears less sensitive than echo in the detection of LVH .
	manualset3
243736	1	422097	7	NULL	NULL	0	NULL	amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of Na represented by NaTC is a function of t : it increases from 1.7 x 10 ( -9 ) mole .
	manualset3
243737	2	422097	7	NULL	NULL	0	NULL	Na 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of Na represented by NaTC is a function of t : it increases from 1.7 x 10 ( -9 ) mole .
	manualset3
243738	3	422097	7	NULL	NULL	0	NULL	NaTC	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of Na represented by NaTC is a function of t : it increases from 1.7 x 10 ( -9 ) mole .
	manualset3
243739	4	422097	7	NULL	NULL	0	NULL	 function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of Na represented by NaTC is a function of t : it increases from 1.7 x 10 ( -9 ) mole .
	manualset3
243740	5	422097	7	NULL	NULL	0	NULL	 t	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of Na represented by NaTC is a function of t : it increases from 1.7 x 10 ( -9 ) mole .
	manualset3
243741	6	422097	7	NULL	NULL	0	NULL	1.7 x 10 ( -9 ) mole	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of Na represented by NaTC is a function of t : it increases from 1.7 x 10 ( -9 ) mole .
	manualset3
243742	1	422098	7	NULL	NULL	0	NULL	Women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Women , conflict , and culture in former Yugoslavia .
	manualset3
243743	2	422098	7	NULL	NULL	0	NULL	conflict	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Women , conflict , and culture in former Yugoslavia .
	manualset3
243744	3	422098	7	NULL	NULL	0	NULL	culture	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Women , conflict , and culture in former Yugoslavia .
	manualset3
243745	4	422098	7	NULL	NULL	0	NULL	Yugoslavia	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Women , conflict , and culture in former Yugoslavia .
	manualset3
243746	1	422099	7	NULL	NULL	0	NULL	rate of decay	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of decay of torque following stretch could not be shown to depend upon stretch variables .
	manualset3
243747	2	422099	7	NULL	NULL	0	NULL	torque	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of decay of torque following stretch could not be shown to depend upon stretch variables .
	manualset3
243748	3	422099	7	NULL	NULL	0	NULL	stretch	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The rate of decay of torque following stretch could not be shown to depend upon stretch variables .
	manualset3
243749	4	422099	7	NULL	NULL	NULL	NULL	stretch variables	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The rate of decay of torque following stretch could not be shown to depend upon stretch variables .
	manualset3
243750	1	422100	7	NULL	NULL	0	NULL	 increased values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Considerably increased values were particularly measured in asymptomatic patients with severe congenital heart disease .
	manualset3
243751	2	422100	7	NULL	NULL	0	NULL	asymptomatic patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Considerably increased values were particularly measured in asymptomatic patients with severe congenital heart disease .
	manualset3
243752	3	422100	7	NULL	NULL	0	NULL	severe congenital heart disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Considerably increased values were particularly measured in asymptomatic patients with severe congenital heart disease .
	manualset3
243753	1	422101	7	NULL	NULL	0	NULL	Future prospective studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Future prospective studies are needed to clarify the risk of developing overt cardiac disease in DM2 and to define prognostic factors .
	manualset3
243754	2	422101	7	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Future prospective studies are needed to clarify the risk of developing overt cardiac disease in DM2 and to define prognostic factors .
	manualset3
243755	3	422101	7	NULL	NULL	0	NULL	overt cardiac disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Future prospective studies are needed to clarify the risk of developing overt cardiac disease in DM2 and to define prognostic factors .
	manualset3
243756	4	422101	7	NULL	NULL	0	NULL	DM2	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Future prospective studies are needed to clarify the risk of developing overt cardiac disease in DM2 and to define prognostic factors .
	manualset3
243757	5	422101	7	NULL	NULL	0	NULL	prognostic factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Future prospective studies are needed to clarify the risk of developing overt cardiac disease in DM2 and to define prognostic factors .
	manualset3
243758	1	422102	7	NULL	NULL	0	NULL	OCT-1 activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	OCT-1 activity was measured in pretherapy blood from chronic myeloid leukemia ( CML ) patients by calculating the difference in IUR of ( ( 14 ) C ) - imatinib with and without OCT-1 inhibition .
	manualset3
243759	2	422102	7	NULL	NULL	0	NULL	pretherapy blood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	OCT-1 activity was measured in pretherapy blood from chronic myeloid leukemia ( CML ) patients by calculating the difference in IUR of ( ( 14 ) C ) - imatinib with and without OCT-1 inhibition .
	manualset3
243760	3	422102	7	NULL	NULL	0	NULL	chronic myeloid leukemia ( CML ) patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	OCT-1 activity was measured in pretherapy blood from chronic myeloid leukemia ( CML ) patients by calculating the difference in IUR of ( ( 14 ) C ) - imatinib with and without OCT-1 inhibition .
	manualset3
243761	4	422102	7	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	OCT-1 activity was measured in pretherapy blood from chronic myeloid leukemia ( CML ) patients by calculating the difference in IUR of ( ( 14 ) C ) - imatinib with and without OCT-1 inhibition .
	manualset3
243762	5	422102	7	NULL	NULL	0	NULL	IUR	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	OCT-1 activity was measured in pretherapy blood from chronic myeloid leukemia ( CML ) patients by calculating the difference in IUR of ( ( 14 ) C ) - imatinib with and without OCT-1 inhibition .
	manualset3
243763	6	422102	7	NULL	NULL	0	NULL	( ( 14 ) C ) - imatinib	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	OCT-1 activity was measured in pretherapy blood from chronic myeloid leukemia ( CML ) patients by calculating the difference in IUR of ( ( 14 ) C ) - imatinib with and without OCT-1 inhibition .
	manualset3
243764	7	422102	7	NULL	NULL	0	NULL	OCT-1 inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	OCT-1 activity was measured in pretherapy blood from chronic myeloid leukemia ( CML ) patients by calculating the difference in IUR of ( ( 14 ) C ) - imatinib with and without OCT-1 inhibition .
	manualset3
243765	1	422103	7	NULL	NULL	0	NULL	evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An evaluation was made of media and tests used for differentiating nonfermenting gram-negative bacteria encountered in medical bacteriology in order to determine those diagnostic procedures most useful in identifying these bacteria .
	manualset3
243766	2	422103	7	NULL	NULL	0	NULL	media 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	An evaluation was made of media and tests used for differentiating nonfermenting gram-negative bacteria encountered in medical bacteriology in order to determine those diagnostic procedures most useful in identifying these bacteria .
	manualset3
243767	3	422103	7	NULL	NULL	0	NULL	tests	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An evaluation was made of media and tests used for differentiating nonfermenting gram-negative bacteria encountered in medical bacteriology in order to determine those diagnostic procedures most useful in identifying these bacteria .
	manualset3
243768	4	422103	7	NULL	NULL	0	NULL	nonfermenting gram-negative bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	An evaluation was made of media and tests used for differentiating nonfermenting gram-negative bacteria encountered in medical bacteriology in order to determine those diagnostic procedures most useful in identifying these bacteria .
	manualset3
243769	5	422103	7	NULL	NULL	0	NULL	medical bacteriology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	An evaluation was made of media and tests used for differentiating nonfermenting gram-negative bacteria encountered in medical bacteriology in order to determine those diagnostic procedures most useful in identifying these bacteria .
	manualset3
243770	6	422103	7	NULL	NULL	0	NULL	diagnostic procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An evaluation was made of media and tests used for differentiating nonfermenting gram-negative bacteria encountered in medical bacteriology in order to determine those diagnostic procedures most useful in identifying these bacteria .
	manualset3
243771	7	422103	7	NULL	NULL	0	NULL	bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	An evaluation was made of media and tests used for differentiating nonfermenting gram-negative bacteria encountered in medical bacteriology in order to determine those diagnostic procedures most useful in identifying these bacteria .
	manualset3
243772	1	422104	7	NULL	NULL	0	NULL	two-step reverse-transcriptase-based polymerase chain reaction ( PCR )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A two-step reverse-transcriptase-based polymerase chain reaction ( PCR ) with nested primer pairs was developed to amplify sensitive and specific cytokeratin-19 ( CK-19 ) mRNA sequences from human breast cancer cells .
	manualset3
243773	2	422104	7	NULL	NULL	0	NULL	nested primer pairs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A two-step reverse-transcriptase-based polymerase chain reaction ( PCR ) with nested primer pairs was developed to amplify sensitive and specific cytokeratin-19 ( CK-19 ) mRNA sequences from human breast cancer cells .
	manualset3
243774	3	422104	7	NULL	NULL	0	NULL	cytokeratin-19 ( CK-19 ) mRNA sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A two-step reverse-transcriptase-based polymerase chain reaction ( PCR ) with nested primer pairs was developed to amplify sensitive and specific cytokeratin-19 ( CK-19 ) mRNA sequences from human breast cancer cells .
	manualset3
243775	4	422104	7	NULL	NULL	0	NULL	human breast cancer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	A two-step reverse-transcriptase-based polymerase chain reaction ( PCR ) with nested primer pairs was developed to amplify sensitive and specific cytokeratin-19 ( CK-19 ) mRNA sequences from human breast cancer cells .
	manualset3
243776	1	422105	7	NULL	NULL	0	NULL	Cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells treated with 0 or 5 Micron choline for 72h detached from the substrate in high numbers ( 58 % of choline deficient cells vs. 1.4 % of choline sufficient cells detached ) exhibited a high incidence of apoptosis ( apoptotic bodies were seen in 55-75 % of cells ; 67-73 % had DNA strand breaks ) , and an absence of mitosis and proliferating cell nuclear antigen ( PCNA ) expression .
	manualset3
243777	2	422105	7	NULL	NULL	0	NULL	0 or 5 Micron	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells treated with 0 or 5 Micron choline for 72h detached from the substrate in high numbers ( 58 % of choline deficient cells vs. 1.4 % of choline sufficient cells detached ) exhibited a high incidence of apoptosis ( apoptotic bodies were seen in 55-75 % of cells ; 67-73 % had DNA strand breaks ) , and an absence of mitosis and proliferating cell nuclear antigen ( PCNA ) expression .
	manualset3
243778	3	422105	7	NULL	NULL	0	NULL	choline	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells treated with 0 or 5 Micron choline for 72h detached from the substrate in high numbers ( 58 % of choline deficient cells vs. 1.4 % of choline sufficient cells detached ) exhibited a high incidence of apoptosis ( apoptotic bodies were seen in 55-75 % of cells ; 67-73 % had DNA strand breaks ) , and an absence of mitosis and proliferating cell nuclear antigen ( PCNA ) expression .
	manualset3
243779	4	422105	7	NULL	NULL	0	NULL	72h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells treated with 0 or 5 Micron choline for 72h detached from the substrate in high numbers ( 58 % of choline deficient cells vs. 1.4 % of choline sufficient cells detached ) exhibited a high incidence of apoptosis ( apoptotic bodies were seen in 55-75 % of cells ; 67-73 % had DNA strand breaks ) , and an absence of mitosis and proliferating cell nuclear antigen ( PCNA ) expression .
	manualset3
243780	5	422105	7	NULL	NULL	0	NULL	substrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells treated with 0 or 5 Micron choline for 72h detached from the substrate in high numbers ( 58 % of choline deficient cells vs. 1.4 % of choline sufficient cells detached ) exhibited a high incidence of apoptosis ( apoptotic bodies were seen in 55-75 % of cells ; 67-73 % had DNA strand breaks ) , and an absence of mitosis and proliferating cell nuclear antigen ( PCNA ) expression .
	manualset3
243781	6	422105	7	NULL	NULL	0	NULL	high numbers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells treated with 0 or 5 Micron choline for 72h detached from the substrate in high numbers ( 58 % of choline deficient cells vs. 1.4 % of choline sufficient cells detached ) exhibited a high incidence of apoptosis ( apoptotic bodies were seen in 55-75 % of cells ; 67-73 % had DNA strand breaks ) , and an absence of mitosis and proliferating cell nuclear antigen ( PCNA ) expression .
	manualset3
243782	7	422105	7	NULL	NULL	0	NULL	58 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells treated with 0 or 5 Micron choline for 72h detached from the substrate in high numbers ( 58 % of choline deficient cells vs. 1.4 % of choline sufficient cells detached ) exhibited a high incidence of apoptosis ( apoptotic bodies were seen in 55-75 % of cells ; 67-73 % had DNA strand breaks ) , and an absence of mitosis and proliferating cell nuclear antigen ( PCNA ) expression .
	manualset3
243783	8	422105	7	NULL	NULL	0	NULL	choline deficient cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells treated with 0 or 5 Micron choline for 72h detached from the substrate in high numbers ( 58 % of choline deficient cells vs. 1.4 % of choline sufficient cells detached ) exhibited a high incidence of apoptosis ( apoptotic bodies were seen in 55-75 % of cells ; 67-73 % had DNA strand breaks ) , and an absence of mitosis and proliferating cell nuclear antigen ( PCNA ) expression .
	manualset3
243784	9	422105	7	NULL	NULL	0	NULL	1.4 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells treated with 0 or 5 Micron choline for 72h detached from the substrate in high numbers ( 58 % of choline deficient cells vs. 1.4 % of choline sufficient cells detached ) exhibited a high incidence of apoptosis ( apoptotic bodies were seen in 55-75 % of cells ; 67-73 % had DNA strand breaks ) , and an absence of mitosis and proliferating cell nuclear antigen ( PCNA ) expression .
	manualset3
243785	10	422105	7	NULL	NULL	0	NULL	choline sufficient cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells treated with 0 or 5 Micron choline for 72h detached from the substrate in high numbers ( 58 % of choline deficient cells vs. 1.4 % of choline sufficient cells detached ) exhibited a high incidence of apoptosis ( apoptotic bodies were seen in 55-75 % of cells ; 67-73 % had DNA strand breaks ) , and an absence of mitosis and proliferating cell nuclear antigen ( PCNA ) expression .
	manualset3
243786	11	422105	7	NULL	NULL	0	NULL	high incidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells treated with 0 or 5 Micron choline for 72h detached from the substrate in high numbers ( 58 % of choline deficient cells vs. 1.4 % of choline sufficient cells detached ) exhibited a high incidence of apoptosis ( apoptotic bodies were seen in 55-75 % of cells ; 67-73 % had DNA strand breaks ) , and an absence of mitosis and proliferating cell nuclear antigen ( PCNA ) expression .
	manualset3
243787	12	422105	7	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells treated with 0 or 5 Micron choline for 72h detached from the substrate in high numbers ( 58 % of choline deficient cells vs. 1.4 % of choline sufficient cells detached ) exhibited a high incidence of apoptosis ( apoptotic bodies were seen in 55-75 % of cells ; 67-73 % had DNA strand breaks ) , and an absence of mitosis and proliferating cell nuclear antigen ( PCNA ) expression .
	manualset3
243788	13	422105	7	NULL	NULL	0	NULL	apoptotic bodies	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells treated with 0 or 5 Micron choline for 72h detached from the substrate in high numbers ( 58 % of choline deficient cells vs. 1.4 % of choline sufficient cells detached ) exhibited a high incidence of apoptosis ( apoptotic bodies were seen in 55-75 % of cells ; 67-73 % had DNA strand breaks ) , and an absence of mitosis and proliferating cell nuclear antigen ( PCNA ) expression .
	manualset3
243789	14	422105	7	NULL	NULL	0	NULL	55-75 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells treated with 0 or 5 Micron choline for 72h detached from the substrate in high numbers ( 58 % of choline deficient cells vs. 1.4 % of choline sufficient cells detached ) exhibited a high incidence of apoptosis ( apoptotic bodies were seen in 55-75 % of cells ; 67-73 % had DNA strand breaks ) , and an absence of mitosis and proliferating cell nuclear antigen ( PCNA ) expression .
	manualset3
243790	15	422105	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells treated with 0 or 5 Micron choline for 72h detached from the substrate in high numbers ( 58 % of choline deficient cells vs. 1.4 % of choline sufficient cells detached ) exhibited a high incidence of apoptosis ( apoptotic bodies were seen in 55-75 % of cells ; 67-73 % had DNA strand breaks ) , and an absence of mitosis and proliferating cell nuclear antigen ( PCNA ) expression .
	manualset3
243791	16	422105	7	NULL	NULL	0	NULL	67-73 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells treated with 0 or 5 Micron choline for 72h detached from the substrate in high numbers ( 58 % of choline deficient cells vs. 1.4 % of choline sufficient cells detached ) exhibited a high incidence of apoptosis ( apoptotic bodies were seen in 55-75 % of cells ; 67-73 % had DNA strand breaks ) , and an absence of mitosis and proliferating cell nuclear antigen ( PCNA ) expression .
	manualset3
243792	17	422105	7	NULL	NULL	0	NULL	DNA strand breaks	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells treated with 0 or 5 Micron choline for 72h detached from the substrate in high numbers ( 58 % of choline deficient cells vs. 1.4 % of choline sufficient cells detached ) exhibited a high incidence of apoptosis ( apoptotic bodies were seen in 55-75 % of cells ; 67-73 % had DNA strand breaks ) , and an absence of mitosis and proliferating cell nuclear antigen ( PCNA ) expression .
	manualset3
243793	18	422105	7	NULL	NULL	0	NULL	 absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells treated with 0 or 5 Micron choline for 72h detached from the substrate in high numbers ( 58 % of choline deficient cells vs. 1.4 % of choline sufficient cells detached ) exhibited a high incidence of apoptosis ( apoptotic bodies were seen in 55-75 % of cells ; 67-73 % had DNA strand breaks ) , and an absence of mitosis and proliferating cell nuclear antigen ( PCNA ) expression .
	manualset3
243794	19	422105	7	NULL	NULL	0	NULL	mitosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells treated with 0 or 5 Micron choline for 72h detached from the substrate in high numbers ( 58 % of choline deficient cells vs. 1.4 % of choline sufficient cells detached ) exhibited a high incidence of apoptosis ( apoptotic bodies were seen in 55-75 % of cells ; 67-73 % had DNA strand breaks ) , and an absence of mitosis and proliferating cell nuclear antigen ( PCNA ) expression .
	manualset3
243795	20	422105	7	NULL	NULL	0	NULL	proliferating cell nuclear antigen ( PCNA ) expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cells treated with 0 or 5 Micron choline for 72h detached from the substrate in high numbers ( 58 % of choline deficient cells vs. 1.4 % of choline sufficient cells detached ) exhibited a high incidence of apoptosis ( apoptotic bodies were seen in 55-75 % of cells ; 67-73 % had DNA strand breaks ) , and an absence of mitosis and proliferating cell nuclear antigen ( PCNA ) expression .
	manualset3
243796	1	422106	7	NULL	NULL	0	NULL	 injuries 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Their injuries were nontender to palpation .
	manualset3
243797	2	422106	7	NULL	NULL	0	NULL	palpation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Their injuries were nontender to palpation .
	manualset3
243798	1	422107	7	NULL	NULL	0	NULL	 Intra - effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intra - and postoperative effect of different hydroxyethyl starch solutions on the flow properties of the blood and on the oxygen partial pressure of the conjunctiva ) .
	manualset3
243799	2	422107	7	NULL	NULL	0	NULL	postoperative effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intra - and postoperative effect of different hydroxyethyl starch solutions on the flow properties of the blood and on the oxygen partial pressure of the conjunctiva ) .
	manualset3
243800	3	422107	7	NULL	NULL	0	NULL	hydroxyethyl starch solutions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intra - and postoperative effect of different hydroxyethyl starch solutions on the flow properties of the blood and on the oxygen partial pressure of the conjunctiva ) .
	manualset3
243801	4	422107	7	NULL	NULL	0	NULL	flow properties	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intra - and postoperative effect of different hydroxyethyl starch solutions on the flow properties of the blood and on the oxygen partial pressure of the conjunctiva ) .
	manualset3
243802	5	422107	7	NULL	NULL	0	NULL	blood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intra - and postoperative effect of different hydroxyethyl starch solutions on the flow properties of the blood and on the oxygen partial pressure of the conjunctiva ) .
	manualset3
243803	6	422107	7	NULL	NULL	0	NULL	oxygen partial pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intra - and postoperative effect of different hydroxyethyl starch solutions on the flow properties of the blood and on the oxygen partial pressure of the conjunctiva ) .
	manualset3
243804	7	422107	7	NULL	NULL	0	NULL	conjunctiva 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intra - and postoperative effect of different hydroxyethyl starch solutions on the flow properties of the blood and on the oxygen partial pressure of the conjunctiva ) .
	manualset3
243805	1	422108	7	NULL	NULL	0	NULL	Livers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Livers with alcoholic hepatitis or cirrhosis had significantly increased nonextractable GAG .
	manualset3
243806	2	422108	7	NULL	NULL	0	NULL	alcoholic hepatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Livers with alcoholic hepatitis or cirrhosis had significantly increased nonextractable GAG .
	manualset3
243807	3	422108	7	NULL	NULL	0	NULL	cirrhosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Livers with alcoholic hepatitis or cirrhosis had significantly increased nonextractable GAG .
	manualset3
243808	4	422108	7	NULL	NULL	0	NULL	nonextractable GAG	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Livers with alcoholic hepatitis or cirrhosis had significantly increased nonextractable GAG .
	manualset3
243809	1	422109	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This study develops a comprehensive theoretical model to describe the transverse relaxation in perfused tissue caused by intravascular tracers .
	manualset3
243810	2	422109	7	NULL	NULL	0	NULL	comprehensive theoretical model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This study develops a comprehensive theoretical model to describe the transverse relaxation in perfused tissue caused by intravascular tracers .
	manualset3
243811	3	422109	7	NULL	NULL	0	NULL	transverse relaxation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This study develops a comprehensive theoretical model to describe the transverse relaxation in perfused tissue caused by intravascular tracers .
	manualset3
243812	4	422109	7	NULL	NULL	0	NULL	perfused tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	This study develops a comprehensive theoretical model to describe the transverse relaxation in perfused tissue caused by intravascular tracers .
	manualset3
243813	5	422109	7	NULL	NULL	NULL	NULL	intravascular tracers	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This study develops a comprehensive theoretical model to describe the transverse relaxation in perfused tissue caused by intravascular tracers .
	manualset3
243814	1	422110	7	NULL	NULL	0	NULL	examination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An examination of kindred histories of 561 Danish probands who have non-syndromic CP has indicated that neither a multifactorial-threshold model nor a single major locus model is completely compatible with the data .
	manualset3
243815	2	422110	7	NULL	NULL	0	NULL	kindred histories	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An examination of kindred histories of 561 Danish probands who have non-syndromic CP has indicated that neither a multifactorial-threshold model nor a single major locus model is completely compatible with the data .
	manualset3
243816	3	422110	7	NULL	NULL	0	NULL	561 Danish probands	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	An examination of kindred histories of 561 Danish probands who have non-syndromic CP has indicated that neither a multifactorial-threshold model nor a single major locus model is completely compatible with the data .
	manualset3
243817	4	422110	7	NULL	NULL	0	NULL	non-syndromic CP	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	An examination of kindred histories of 561 Danish probands who have non-syndromic CP has indicated that neither a multifactorial-threshold model nor a single major locus model is completely compatible with the data .
	manualset3
243818	5	422110	7	NULL	NULL	0	NULL	multifactorial-threshold model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	An examination of kindred histories of 561 Danish probands who have non-syndromic CP has indicated that neither a multifactorial-threshold model nor a single major locus model is completely compatible with the data .
	manualset3
243819	6	422110	7	NULL	NULL	0	NULL	single major locus model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	An examination of kindred histories of 561 Danish probands who have non-syndromic CP has indicated that neither a multifactorial-threshold model nor a single major locus model is completely compatible with the data .
	manualset3
243820	7	422110	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	An examination of kindred histories of 561 Danish probands who have non-syndromic CP has indicated that neither a multifactorial-threshold model nor a single major locus model is completely compatible with the data .
	manualset3
243821	1	422111	7	NULL	NULL	0	NULL	Protein kinase C isoenzymes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein kinase C isoenzymes : a review of their structure , regulation and role in regulating airways smooth muscle tone and mitogenesis .
	manualset3
243822	2	422111	7	NULL	NULL	0	NULL	review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein kinase C isoenzymes : a review of their structure , regulation and role in regulating airways smooth muscle tone and mitogenesis .
	manualset3
243823	3	422111	7	NULL	NULL	0	NULL	structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein kinase C isoenzymes : a review of their structure , regulation and role in regulating airways smooth muscle tone and mitogenesis .
	manualset3
243824	4	422111	7	NULL	NULL	0	NULL	regulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein kinase C isoenzymes : a review of their structure , regulation and role in regulating airways smooth muscle tone and mitogenesis .
	manualset3
243825	5	422111	7	NULL	NULL	0	NULL	role 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein kinase C isoenzymes : a review of their structure , regulation and role in regulating airways smooth muscle tone and mitogenesis .
	manualset3
243826	6	422111	7	NULL	NULL	0	NULL	airways smooth muscle tone	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein kinase C isoenzymes : a review of their structure , regulation and role in regulating airways smooth muscle tone and mitogenesis .
	manualset3
243827	7	422111	7	NULL	NULL	0	NULL	mitogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Protein kinase C isoenzymes : a review of their structure , regulation and role in regulating airways smooth muscle tone and mitogenesis .
	manualset3
243828	1	422112	7	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional data are provided on Ecuador 's people , government , economy , international affiliations , history , political conditions , principal government officials , foreign relations , and bilateral relations with the United States .
	manualset3
243829	2	422112	7	NULL	NULL	0	NULL	Ecuador 's people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional data are provided on Ecuador 's people , government , economy , international affiliations , history , political conditions , principal government officials , foreign relations , and bilateral relations with the United States .
	manualset3
243830	3	422112	7	NULL	NULL	0	NULL	government 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional data are provided on Ecuador 's people , government , economy , international affiliations , history , political conditions , principal government officials , foreign relations , and bilateral relations with the United States .
	manualset3
243831	4	422112	7	NULL	NULL	0	NULL	economy	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional data are provided on Ecuador 's people , government , economy , international affiliations , history , political conditions , principal government officials , foreign relations , and bilateral relations with the United States .
	manualset3
243832	5	422112	7	NULL	NULL	0	NULL	international affiliations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional data are provided on Ecuador 's people , government , economy , international affiliations , history , political conditions , principal government officials , foreign relations , and bilateral relations with the United States .
	manualset3
243833	6	422112	7	NULL	NULL	0	NULL	history	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional data are provided on Ecuador 's people , government , economy , international affiliations , history , political conditions , principal government officials , foreign relations , and bilateral relations with the United States .
	manualset3
243834	7	422112	7	NULL	NULL	0	NULL	political conditions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional data are provided on Ecuador 's people , government , economy , international affiliations , history , political conditions , principal government officials , foreign relations , and bilateral relations with the United States .
	manualset3
243835	8	422112	7	NULL	NULL	0	NULL	principal government officials	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional data are provided on Ecuador 's people , government , economy , international affiliations , history , political conditions , principal government officials , foreign relations , and bilateral relations with the United States .
	manualset3
243836	9	422112	7	NULL	NULL	0	NULL	foreign relations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional data are provided on Ecuador 's people , government , economy , international affiliations , history , political conditions , principal government officials , foreign relations , and bilateral relations with the United States .
	manualset3
243837	10	422112	7	NULL	NULL	0	NULL	bilateral relations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional data are provided on Ecuador 's people , government , economy , international affiliations , history , political conditions , principal government officials , foreign relations , and bilateral relations with the United States .
	manualset3
243838	11	422112	7	NULL	NULL	0	NULL	United States	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Additional data are provided on Ecuador 's people , government , economy , international affiliations , history , political conditions , principal government officials , foreign relations , and bilateral relations with the United States .
	manualset3
243839	1	422113	7	NULL	NULL	0	NULL	 leucocyte migration inhibition ( LMI )  leucocyte migration inhibition ( LMI ) 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The leucocyte migration inhibition ( LMI ) was determined in an assay after in vitro challenge with beta-lactoglobulin .
	manualset3
243840	2	422113	7	NULL	NULL	0	NULL	assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The leucocyte migration inhibition ( LMI ) was determined in an assay after in vitro challenge with beta-lactoglobulin .
	manualset3
243841	3	422113	7	NULL	NULL	0	NULL	in vitro challenge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The leucocyte migration inhibition ( LMI ) was determined in an assay after in vitro challenge with beta-lactoglobulin .
	manualset3
243842	4	422113	7	NULL	NULL	0	NULL	beta-lactoglobulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The leucocyte migration inhibition ( LMI ) was determined in an assay after in vitro challenge with beta-lactoglobulin .
	manualset3
243843	1	422114	7	NULL	NULL	0	NULL	Vegetable foreign body	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Vegetable foreign body in the testis ) .
	manualset3
243844	2	422114	7	NULL	NULL	0	NULL	testis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Vegetable foreign body in the testis ) .
	manualset3
243845	1	422115	7	NULL	NULL	0	NULL	nimodipine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of nimodipine , a dihydropyridine calcium antagonist , to reduce the daily dose of oral morphine in cancer patients who had developed dose escalation , was tested in 54 patients under randomized , double-blind , placebo-controlled conditions .
	manualset3
243846	2	422115	7	NULL	NULL	0	NULL	dihydropyridine calcium antagonist	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of nimodipine , a dihydropyridine calcium antagonist , to reduce the daily dose of oral morphine in cancer patients who had developed dose escalation , was tested in 54 patients under randomized , double-blind , placebo-controlled conditions .
	manualset3
243847	3	422115	7	NULL	NULL	0	NULL	 daily dose 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of nimodipine , a dihydropyridine calcium antagonist , to reduce the daily dose of oral morphine in cancer patients who had developed dose escalation , was tested in 54 patients under randomized , double-blind , placebo-controlled conditions .
	manualset3
243848	4	422115	7	NULL	NULL	0	NULL	oral morphine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of nimodipine , a dihydropyridine calcium antagonist , to reduce the daily dose of oral morphine in cancer patients who had developed dose escalation , was tested in 54 patients under randomized , double-blind , placebo-controlled conditions .
	manualset3
243849	5	422115	7	NULL	NULL	0	NULL	cancer patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of nimodipine , a dihydropyridine calcium antagonist , to reduce the daily dose of oral morphine in cancer patients who had developed dose escalation , was tested in 54 patients under randomized , double-blind , placebo-controlled conditions .
	manualset3
243850	6	422115	7	NULL	NULL	0	NULL	dose escalation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of nimodipine , a dihydropyridine calcium antagonist , to reduce the daily dose of oral morphine in cancer patients who had developed dose escalation , was tested in 54 patients under randomized , double-blind , placebo-controlled conditions .
	manualset3
243851	7	422115	7	NULL	NULL	0	NULL	54 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of nimodipine , a dihydropyridine calcium antagonist , to reduce the daily dose of oral morphine in cancer patients who had developed dose escalation , was tested in 54 patients under randomized , double-blind , placebo-controlled conditions .
	manualset3
243852	8	422115	7	NULL	NULL	0	NULL	placebo-controlled conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of nimodipine , a dihydropyridine calcium antagonist , to reduce the daily dose of oral morphine in cancer patients who had developed dose escalation , was tested in 54 patients under randomized , double-blind , placebo-controlled conditions .
	manualset3
244695	9	422115	7	NULL	NULL	0	NULL	randomized conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of nimodipine , a dihydropyridine calcium antagonist , to reduce the daily dose of oral morphine in cancer patients who had developed dose escalation , was tested in 54 patients under randomized , double-blind , placebo-controlled conditions .
	manualset3
244696	10	422115	7	NULL	NULL	0	NULL	double-blind conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of nimodipine , a dihydropyridine calcium antagonist , to reduce the daily dose of oral morphine in cancer patients who had developed dose escalation , was tested in 54 patients under randomized , double-blind , placebo-controlled conditions .
	manualset3
247476	11	422115	7	NULL	NULL	0	NULL	 ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The ability of nimodipine , a dihydropyridine calcium antagonist , to reduce the daily dose of oral morphine in cancer patients who had developed dose escalation , was tested in 54 patients under randomized , double-blind , placebo-controlled conditions .
	manualset3
243853	1	422116	7	NULL	NULL	0	NULL	 numbers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The numbers of horses at individual stables were too small to draw conclusions at each stable , but whereas efficacies greater than 85 per cent were recorded for pyrantel at 26 of 27 stables , the corresponding figure for fenbendazole was five of 27 .
	manualset3
243854	2	422116	7	NULL	NULL	0	NULL	horses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The numbers of horses at individual stables were too small to draw conclusions at each stable , but whereas efficacies greater than 85 per cent were recorded for pyrantel at 26 of 27 stables , the corresponding figure for fenbendazole was five of 27 .
	manualset3
243855	3	422116	7	NULL	NULL	0	NULL	 individual stables	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The numbers of horses at individual stables were too small to draw conclusions at each stable , but whereas efficacies greater than 85 per cent were recorded for pyrantel at 26 of 27 stables , the corresponding figure for fenbendazole was five of 27 .
	manualset3
243856	4	422116	7	NULL	NULL	0	NULL	conclusions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The numbers of horses at individual stables were too small to draw conclusions at each stable , but whereas efficacies greater than 85 per cent were recorded for pyrantel at 26 of 27 stables , the corresponding figure for fenbendazole was five of 27 .
	manualset3
243857	5	422116	7	NULL	NULL	0	NULL	85 per cent 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The numbers of horses at individual stables were too small to draw conclusions at each stable , but whereas efficacies greater than 85 per cent were recorded for pyrantel at 26 of 27 stables , the corresponding figure for fenbendazole was five of 27 .
	manualset3
243858	6	422116	7	NULL	NULL	0	NULL	 pyrantel	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The numbers of horses at individual stables were too small to draw conclusions at each stable , but whereas efficacies greater than 85 per cent were recorded for pyrantel at 26 of 27 stables , the corresponding figure for fenbendazole was five of 27 .
	manualset3
243859	7	422116	7	NULL	NULL	0	NULL	26	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The numbers of horses at individual stables were too small to draw conclusions at each stable , but whereas efficacies greater than 85 per cent were recorded for pyrantel at 26 of 27 stables , the corresponding figure for fenbendazole was five of 27 .
	manualset3
243860	8	422116	7	NULL	NULL	0	NULL	 27 stables	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The numbers of horses at individual stables were too small to draw conclusions at each stable , but whereas efficacies greater than 85 per cent were recorded for pyrantel at 26 of 27 stables , the corresponding figure for fenbendazole was five of 27 .
	manualset3
243861	9	422116	7	NULL	NULL	0	NULL	corresponding figure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The numbers of horses at individual stables were too small to draw conclusions at each stable , but whereas efficacies greater than 85 per cent were recorded for pyrantel at 26 of 27 stables , the corresponding figure for fenbendazole was five of 27 .
	manualset3
243862	10	422116	7	NULL	NULL	0	NULL	fenbendazole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The numbers of horses at individual stables were too small to draw conclusions at each stable , but whereas efficacies greater than 85 per cent were recorded for pyrantel at 26 of 27 stables , the corresponding figure for fenbendazole was five of 27 .
	manualset3
243863	11	422116	7	NULL	NULL	0	NULL	 five	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The numbers of horses at individual stables were too small to draw conclusions at each stable , but whereas efficacies greater than 85 per cent were recorded for pyrantel at 26 of 27 stables , the corresponding figure for fenbendazole was five of 27 .
	manualset3
243864	12	422116	7	NULL	NULL	0	NULL	 27	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The numbers of horses at individual stables were too small to draw conclusions at each stable , but whereas efficacies greater than 85 per cent were recorded for pyrantel at 26 of 27 stables , the corresponding figure for fenbendazole was five of 27 .
	manualset3
243865	13	422116	7	NULL	NULL	0	NULL	stable	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	The numbers of horses at individual stables were too small to draw conclusions at each stable , but whereas efficacies greater than 85 per cent were recorded for pyrantel at 26 of 27 stables , the corresponding figure for fenbendazole was five of 27 .
	manualset3
243866	1	422117	7	NULL	NULL	0	NULL	 Psychiatric aspect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Psychiatric and psychological aspects of pharmacotherapy in personality disorders ( author 's transl ) ) .
	manualset3
243867	2	422117	7	NULL	NULL	0	NULL	psychological aspects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Psychiatric and psychological aspects of pharmacotherapy in personality disorders ( author 's transl ) ) .
	manualset3
243868	3	422117	7	NULL	NULL	0	NULL	pharmacotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Psychiatric and psychological aspects of pharmacotherapy in personality disorders ( author 's transl ) ) .
	manualset3
243869	4	422117	7	NULL	NULL	0	NULL	personality disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Psychiatric and psychological aspects of pharmacotherapy in personality disorders ( author 's transl ) ) .
	manualset3
243870	5	422117	7	NULL	NULL	0	NULL	author 's transl	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Psychiatric and psychological aspects of pharmacotherapy in personality disorders ( author 's transl ) ) .
	manualset3
243871	1	422118	7	NULL	NULL	0	NULL	 average	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On average , the hippocampus , a forebrain structure that processes spatial information , is larger in homing pigeons compared to other non-homing pigeon breeds or their wild ancestor , the rock dove .
	manualset3
243872	2	422118	7	NULL	NULL	0	NULL	hippocampus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	On average , the hippocampus , a forebrain structure that processes spatial information , is larger in homing pigeons compared to other non-homing pigeon breeds or their wild ancestor , the rock dove .
	manualset3
243873	3	422118	7	NULL	NULL	0	NULL	forebrain structure	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	On average , the hippocampus , a forebrain structure that processes spatial information , is larger in homing pigeons compared to other non-homing pigeon breeds or their wild ancestor , the rock dove .
	manualset3
243874	4	422118	7	NULL	NULL	0	NULL	spatial information	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On average , the hippocampus , a forebrain structure that processes spatial information , is larger in homing pigeons compared to other non-homing pigeon breeds or their wild ancestor , the rock dove .
	manualset3
243875	5	422118	7	NULL	NULL	NULL	NULL	homing pigeons	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On average , the hippocampus , a forebrain structure that processes spatial information , is larger in homing pigeons compared to other non-homing pigeon breeds or their wild ancestor , the rock dove .
	manualset3
243876	6	422118	7	NULL	NULL	0	NULL	non-homing pigeon breeds	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On average , the hippocampus , a forebrain structure that processes spatial information , is larger in homing pigeons compared to other non-homing pigeon breeds or their wild ancestor , the rock dove .
	manualset3
243877	7	422118	7	NULL	NULL	0	NULL	 wild ancestor	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On average , the hippocampus , a forebrain structure that processes spatial information , is larger in homing pigeons compared to other non-homing pigeon breeds or their wild ancestor , the rock dove .
	manualset3
243878	8	422118	7	NULL	NULL	0	NULL	rock dove	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	On average , the hippocampus , a forebrain structure that processes spatial information , is larger in homing pigeons compared to other non-homing pigeon breeds or their wild ancestor , the rock dove .
	manualset3
243879	1	422119	7	NULL	NULL	0	NULL	 providers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Few providers ( 18.1 % ) reported high levels of confidence in their ability to counsel smoking patients .
	manualset3
243880	2	422119	7	NULL	NULL	0	NULL	18.1 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Few providers ( 18.1 % ) reported high levels of confidence in their ability to counsel smoking patients .
	manualset3
243881	3	422119	7	NULL	NULL	0	NULL	high levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Few providers ( 18.1 % ) reported high levels of confidence in their ability to counsel smoking patients .
	manualset3
243882	4	422119	7	NULL	NULL	0	NULL	confidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Few providers ( 18.1 % ) reported high levels of confidence in their ability to counsel smoking patients .
	manualset3
243883	5	422119	7	NULL	NULL	0	NULL	smoking patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Few providers ( 18.1 % ) reported high levels of confidence in their ability to counsel smoking patients .
	manualset3
243884	1	422120	7	NULL	NULL	0	NULL	examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An examination of nucleus accumbens cell firing during extinction and reinstatement of water reinforcement behavior in rats .
	manualset3
243885	2	422120	7	NULL	NULL	0	NULL	nucleus accumbens cell firing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An examination of nucleus accumbens cell firing during extinction and reinstatement of water reinforcement behavior in rats .
	manualset3
243886	3	422120	7	NULL	NULL	0	NULL	extinction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An examination of nucleus accumbens cell firing during extinction and reinstatement of water reinforcement behavior in rats .
	manualset3
243887	4	422120	7	NULL	NULL	0	NULL	 reinstatement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An examination of nucleus accumbens cell firing during extinction and reinstatement of water reinforcement behavior in rats .
	manualset3
243888	5	422120	7	NULL	NULL	0	NULL	water reinforcement behavior	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An examination of nucleus accumbens cell firing during extinction and reinstatement of water reinforcement behavior in rats .
	manualset3
243889	6	422120	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	An examination of nucleus accumbens cell firing during extinction and reinstatement of water reinforcement behavior in rats .
	manualset3
243890	1	422121	7	NULL	NULL	NULL	NULL	CD1d 	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	CD1d is a key antigen-presenting molecule involved in the selection and activation of a highly conserved T cell subset known as NK T cells .
	manualset3
243891	2	422121	7	NULL	NULL	0	NULL	antigen-presenting molecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	CD1d is a key antigen-presenting molecule involved in the selection and activation of a highly conserved T cell subset known as NK T cells .
	manualset3
243892	3	422121	7	NULL	NULL	0	NULL	selection	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	CD1d is a key antigen-presenting molecule involved in the selection and activation of a highly conserved T cell subset known as NK T cells .
	manualset3
243893	4	422121	7	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	CD1d is a key antigen-presenting molecule involved in the selection and activation of a highly conserved T cell subset known as NK T cells .
	manualset3
243894	5	422121	7	NULL	NULL	0	NULL	highly conserved T cell subset	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	CD1d is a key antigen-presenting molecule involved in the selection and activation of a highly conserved T cell subset known as NK T cells .
	manualset3
243895	6	422121	7	NULL	NULL	0	NULL	NK T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	CD1d is a key antigen-presenting molecule involved in the selection and activation of a highly conserved T cell subset known as NK T cells .
	manualset3
243896	1	422122	7	NULL	NULL	0	NULL	article	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This article is devoted to the new method for the determination of basal metabolism using 13C-bicarbonate breath test compared to the method of Harris-Benedict in healthy and patients with impaired thyroid function .
	manualset3
243897	2	422122	7	NULL	NULL	0	NULL	new method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This article is devoted to the new method for the determination of basal metabolism using 13C-bicarbonate breath test compared to the method of Harris-Benedict in healthy and patients with impaired thyroid function .
	manualset3
243898	3	422122	7	NULL	NULL	0	NULL	determination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This article is devoted to the new method for the determination of basal metabolism using 13C-bicarbonate breath test compared to the method of Harris-Benedict in healthy and patients with impaired thyroid function .
	manualset3
243899	4	422122	7	NULL	NULL	0	NULL	 basal metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This article is devoted to the new method for the determination of basal metabolism using 13C-bicarbonate breath test compared to the method of Harris-Benedict in healthy and patients with impaired thyroid function .
	manualset3
243900	5	422122	7	NULL	NULL	0	NULL	13C-bicarbonate breath test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article is devoted to the new method for the determination of basal metabolism using 13C-bicarbonate breath test compared to the method of Harris-Benedict in healthy and patients with impaired thyroid function .
	manualset3
243901	6	422122	7	NULL	NULL	0	NULL	 method 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This article is devoted to the new method for the determination of basal metabolism using 13C-bicarbonate breath test compared to the method of Harris-Benedict in healthy and patients with impaired thyroid function .
	manualset3
243902	7	422122	7	NULL	NULL	0	NULL	Harris-Benedict	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This article is devoted to the new method for the determination of basal metabolism using 13C-bicarbonate breath test compared to the method of Harris-Benedict in healthy and patients with impaired thyroid function .
	manualset3
243903	8	422122	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This article is devoted to the new method for the determination of basal metabolism using 13C-bicarbonate breath test compared to the method of Harris-Benedict in healthy and patients with impaired thyroid function .
	manualset3
243904	9	422122	7	NULL	NULL	0	NULL	impaired thyroid function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This article is devoted to the new method for the determination of basal metabolism using 13C-bicarbonate breath test compared to the method of Harris-Benedict in healthy and patients with impaired thyroid function .
	manualset3
243905	1	422123	7	NULL	NULL	0	NULL	 work	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This work tested the hypothesis that a stereospecific topical formulation could be used to engineer differential permeation rates for each enantiomer of an applied racemate across human skin in vitro .
	manualset3
243906	2	422123	7	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This work tested the hypothesis that a stereospecific topical formulation could be used to engineer differential permeation rates for each enantiomer of an applied racemate across human skin in vitro .
	manualset3
243907	3	422123	7	NULL	NULL	0	NULL	stereospecific topical formulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This work tested the hypothesis that a stereospecific topical formulation could be used to engineer differential permeation rates for each enantiomer of an applied racemate across human skin in vitro .
	manualset3
243908	4	422123	7	NULL	NULL	0	NULL	differential permeation rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This work tested the hypothesis that a stereospecific topical formulation could be used to engineer differential permeation rates for each enantiomer of an applied racemate across human skin in vitro .
	manualset3
243909	5	422123	7	NULL	NULL	0	NULL	enantiomer	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	This work tested the hypothesis that a stereospecific topical formulation could be used to engineer differential permeation rates for each enantiomer of an applied racemate across human skin in vitro .
	manualset3
243910	6	422123	7	NULL	NULL	0	NULL	applied racemate	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	This work tested the hypothesis that a stereospecific topical formulation could be used to engineer differential permeation rates for each enantiomer of an applied racemate across human skin in vitro .
	manualset3
243911	7	422123	7	NULL	NULL	0	NULL	human skin 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	This work tested the hypothesis that a stereospecific topical formulation could be used to engineer differential permeation rates for each enantiomer of an applied racemate across human skin in vitro .
	manualset3
243912	1	422124	7	NULL	NULL	0	NULL	Ultratrace analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultratrace analysis of nine macrolides , including tulathromycin A ( Draxxin ) , in edible animal tissues with minicolumn liquid chromatography tandem mass spectrometry .
	manualset3
243913	2	422124	7	NULL	NULL	0	NULL	nine macrolides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultratrace analysis of nine macrolides , including tulathromycin A ( Draxxin ) , in edible animal tissues with minicolumn liquid chromatography tandem mass spectrometry .
	manualset3
243914	3	422124	7	NULL	NULL	0	NULL	 tulathromycin A ( Draxxin )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultratrace analysis of nine macrolides , including tulathromycin A ( Draxxin ) , in edible animal tissues with minicolumn liquid chromatography tandem mass spectrometry .
	manualset3
243915	4	422124	7	NULL	NULL	0	NULL	edible animal tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultratrace analysis of nine macrolides , including tulathromycin A ( Draxxin ) , in edible animal tissues with minicolumn liquid chromatography tandem mass spectrometry .
	manualset3
243916	5	422124	7	NULL	NULL	0	NULL	minicolumn liquid chromatography tandem mass spectrometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ultratrace analysis of nine macrolides , including tulathromycin A ( Draxxin ) , in edible animal tissues with minicolumn liquid chromatography tandem mass spectrometry .
	manualset3
243917	1	422125	7	NULL	NULL	0	NULL	eRF1 molecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The eRF1 molecule bound to the ribosome undergone substantial conformational changes resulting in the mutual configuration of the N - and M-domains similar to tRNA shape .
	manualset3
243918	2	422125	7	NULL	NULL	0	NULL	ribosome	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The eRF1 molecule bound to the ribosome undergone substantial conformational changes resulting in the mutual configuration of the N - and M-domains similar to tRNA shape .
	manualset3
243919	3	422125	7	NULL	NULL	0	NULL	conformational changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The eRF1 molecule bound to the ribosome undergone substantial conformational changes resulting in the mutual configuration of the N - and M-domains similar to tRNA shape .
	manualset3
243920	4	422125	7	NULL	NULL	0	NULL	mutual configuration	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The eRF1 molecule bound to the ribosome undergone substantial conformational changes resulting in the mutual configuration of the N - and M-domains similar to tRNA shape .
	manualset3
243921	5	422125	7	NULL	NULL	0	NULL	N -domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The eRF1 molecule bound to the ribosome undergone substantial conformational changes resulting in the mutual configuration of the N - and M-domains similar to tRNA shape .
	manualset3
243922	6	422125	7	NULL	NULL	0	NULL	M-domains 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	The eRF1 molecule bound to the ribosome undergone substantial conformational changes resulting in the mutual configuration of the N - and M-domains similar to tRNA shape .
	manualset3
243923	7	422125	7	NULL	NULL	0	NULL	tRNA shape	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The eRF1 molecule bound to the ribosome undergone substantial conformational changes resulting in the mutual configuration of the N - and M-domains similar to tRNA shape .
	manualset3
243924	1	422126	7	NULL	NULL	0	NULL	case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of the collagen profile , the pepsin-solubilized collagen content and its relative percentage to the total collagen were significantly higher than in the control .
	manualset3
243925	2	422126	7	NULL	NULL	0	NULL	collagen profile	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of the collagen profile , the pepsin-solubilized collagen content and its relative percentage to the total collagen were significantly higher than in the control .
	manualset3
243926	3	422126	7	NULL	NULL	0	NULL	 pepsin-solubilized collagen content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of the collagen profile , the pepsin-solubilized collagen content and its relative percentage to the total collagen were significantly higher than in the control .
	manualset3
243927	4	422126	7	NULL	NULL	0	NULL	relative percentage	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of the collagen profile , the pepsin-solubilized collagen content and its relative percentage to the total collagen were significantly higher than in the control .
	manualset3
243928	5	422126	7	NULL	NULL	0	NULL	 total collagen	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of the collagen profile , the pepsin-solubilized collagen content and its relative percentage to the total collagen were significantly higher than in the control .
	manualset3
243929	6	422126	7	NULL	NULL	0	NULL	control	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	In the case of the collagen profile , the pepsin-solubilized collagen content and its relative percentage to the total collagen were significantly higher than in the control .
	manualset3
243930	1	422127	7	NULL	NULL	0	NULL	Relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between magnetic resonance imaging and molecular pathology in patients with glioblastoma multiforme .
	manualset3
243931	2	422127	7	NULL	NULL	0	NULL	magnetic resonance imaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between magnetic resonance imaging and molecular pathology in patients with glioblastoma multiforme .
	manualset3
243932	3	422127	7	NULL	NULL	0	NULL	molecular pathology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between magnetic resonance imaging and molecular pathology in patients with glioblastoma multiforme .
	manualset3
243933	4	422127	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between magnetic resonance imaging and molecular pathology in patients with glioblastoma multiforme .
	manualset3
243934	5	422127	7	NULL	NULL	0	NULL	glioblastoma multiforme	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Relationship between magnetic resonance imaging and molecular pathology in patients with glioblastoma multiforme .
	manualset3
243935	1	422128	7	NULL	NULL	0	NULL	 result	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This result suggested that the region around the boundary of 11q22.3-q23 .1 was intact in this patient .
	manualset3
243936	2	422128	7	NULL	NULL	0	NULL	region	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	This result suggested that the region around the boundary of 11q22.3-q23 .1 was intact in this patient .
	manualset3
243937	3	422128	7	NULL	NULL	0	NULL	boundary	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	This result suggested that the region around the boundary of 11q22.3-q23 .1 was intact in this patient .
	manualset3
243938	4	422128	7	NULL	NULL	0	NULL	11q22.3-q23 .1	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	This result suggested that the region around the boundary of 11q22.3-q23 .1 was intact in this patient .
	manualset3
243939	5	422128	7	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	This result suggested that the region around the boundary of 11q22.3-q23 .1 was intact in this patient .
	manualset3
243940	1	422129	7	NULL	NULL	0	NULL	Farnesyltransferase inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Farnesyltransferase inhibitors versus Ras inhibitors .
	manualset3
243941	2	422129	7	NULL	NULL	0	NULL	Ras inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Farnesyltransferase inhibitors versus Ras inhibitors .
	manualset3
243942	1	422130	7	NULL	NULL	0	NULL	Stroke volume	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stroke volume and cardiac output ( SV , CO ) and indexes ( SI , CI ) were determined by impedance cardiography .
	manualset3
243943	2	422130	7	NULL	NULL	0	NULL	cardiac output ( SV , CO )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Stroke volume and cardiac output ( SV , CO ) and indexes ( SI , CI ) were determined by impedance cardiography .
	manualset3
243944	3	422130	7	NULL	NULL	0	NULL	indexes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stroke volume and cardiac output ( SV , CO ) and indexes ( SI , CI ) were determined by impedance cardiography .
	manualset3
243945	4	422130	7	NULL	NULL	0	NULL	 SI	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stroke volume and cardiac output ( SV , CO ) and indexes ( SI , CI ) were determined by impedance cardiography .
	manualset3
243946	5	422130	7	NULL	NULL	0	NULL	CI	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Stroke volume and cardiac output ( SV , CO ) and indexes ( SI , CI ) were determined by impedance cardiography .
	manualset3
243947	6	422130	7	NULL	NULL	0	NULL	impedance cardiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Stroke volume and cardiac output ( SV , CO ) and indexes ( SI , CI ) were determined by impedance cardiography .
	manualset3
243948	1	422131	7	NULL	NULL	0	NULL	different flexibility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The different flexibility of c-Src and c-Abl kinases regulates the accessibility of a druggable inactive conformation .
	manualset3
243962	2	422131	7	NULL	NULL	0	NULL	c-Src 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The different flexibility of c-Src and c-Abl kinases regulates the accessibility of a druggable inactive conformation .
	manualset3
243963	3	422131	7	NULL	NULL	0	NULL	c-Abl kinases	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The different flexibility of c-Src and c-Abl kinases regulates the accessibility of a druggable inactive conformation .
	manualset3
243964	4	422131	7	NULL	NULL	0	NULL	accessibility	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The different flexibility of c-Src and c-Abl kinases regulates the accessibility of a druggable inactive conformation .
	manualset3
243965	5	422131	7	NULL	NULL	0	NULL	druggable inactive conformation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The different flexibility of c-Src and c-Abl kinases regulates the accessibility of a druggable inactive conformation .
	manualset3
243966	1	422132	7	NULL	NULL	0	NULL	Ribozyme cleavage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ribozyme cleavage of a 2 , 5-phosphodiester linkage : mechanism and a restricted divalent metal-ion requirement .
	manualset3
243967	2	422132	7	NULL	NULL	0	NULL	2 , 5-phosphodiester linkage	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ribozyme cleavage of a 2 , 5-phosphodiester linkage : mechanism and a restricted divalent metal-ion requirement .
	manualset3
243968	3	422132	7	NULL	NULL	0	NULL	mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ribozyme cleavage of a 2 , 5-phosphodiester linkage : mechanism and a restricted divalent metal-ion requirement .
	manualset3
243969	4	422132	7	NULL	NULL	0	NULL	divalent metal-ion requirement	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ribozyme cleavage of a 2 , 5-phosphodiester linkage : mechanism and a restricted divalent metal-ion requirement .
	manualset3
243970	1	422133	7	NULL	NULL	0	NULL	high-frequency words	Language												NULL		0	NULL	NULL	NULL	NULL	NULL	This has been attributed to high-frequency words ' being better represented and providing more effective support to a redintegration process at retrieval ( C. Hulme et al. , 1997 ) .
	manualset3
243971	2	422133	7	NULL	NULL	0	NULL	redintegration process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This has been attributed to high-frequency words ' being better represented and providing more effective support to a redintegration process at retrieval ( C. Hulme et al. , 1997 ) .
	manualset3
243972	3	422133	7	NULL	NULL	0	NULL	retrieval	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This has been attributed to high-frequency words ' being better represented and providing more effective support to a redintegration process at retrieval ( C. Hulme et al. , 1997 ) .
	manualset3
243973	4	422133	7	NULL	NULL	0	NULL	C. Hulme et al. ,	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	This has been attributed to high-frequency words ' being better represented and providing more effective support to a redintegration process at retrieval ( C. Hulme et al. , 1997 ) .
	manualset3
243974	5	422133	7	NULL	NULL	0	NULL	1997	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	This has been attributed to high-frequency words ' being better represented and providing more effective support to a redintegration process at retrieval ( C. Hulme et al. , 1997 ) .
	manualset3
245780	6	422133	7	NULL	NULL	0	NULL	effective support	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This has been attributed to high-frequency words ' being better represented and providing more effective support to a redintegration process at retrieval ( C. Hulme et al. , 1997 ) .
	manualset3
243975	1	422134	7	NULL	NULL	0	NULL	sum of area	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the sum of area under the concentration-time profile ( AUC ) ( BDCRB ) and AUC ( prodrug ) after l-Asp-BDCRB administration was roughly 3-fold greater than AUC ( BDCRB ) after BDCRB administration , suggesting that a reservoir of prodrug was delivered in addition to parent drug .
	manualset3
243976	2	422134	7	NULL	NULL	0	NULL	concentration-time profile ( AUC )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the sum of area under the concentration-time profile ( AUC ) ( BDCRB ) and AUC ( prodrug ) after l-Asp-BDCRB administration was roughly 3-fold greater than AUC ( BDCRB ) after BDCRB administration , suggesting that a reservoir of prodrug was delivered in addition to parent drug .
	manualset3
243977	3	422134	7	NULL	NULL	0	NULL	BDCRB	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the sum of area under the concentration-time profile ( AUC ) ( BDCRB ) and AUC ( prodrug ) after l-Asp-BDCRB administration was roughly 3-fold greater than AUC ( BDCRB ) after BDCRB administration , suggesting that a reservoir of prodrug was delivered in addition to parent drug .
	manualset3
243978	4	422134	7	NULL	NULL	0	NULL	AUC 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the sum of area under the concentration-time profile ( AUC ) ( BDCRB ) and AUC ( prodrug ) after l-Asp-BDCRB administration was roughly 3-fold greater than AUC ( BDCRB ) after BDCRB administration , suggesting that a reservoir of prodrug was delivered in addition to parent drug .
	manualset3
243979	5	422134	7	NULL	NULL	0	NULL	prodrug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the sum of area under the concentration-time profile ( AUC ) ( BDCRB ) and AUC ( prodrug ) after l-Asp-BDCRB administration was roughly 3-fold greater than AUC ( BDCRB ) after BDCRB administration , suggesting that a reservoir of prodrug was delivered in addition to parent drug .
	manualset3
243980	6	422134	7	NULL	NULL	0	NULL	 l-Asp-BDCRB administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the sum of area under the concentration-time profile ( AUC ) ( BDCRB ) and AUC ( prodrug ) after l-Asp-BDCRB administration was roughly 3-fold greater than AUC ( BDCRB ) after BDCRB administration , suggesting that a reservoir of prodrug was delivered in addition to parent drug .
	manualset3
243981	7	422134	7	NULL	NULL	0	NULL	3-fold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the sum of area under the concentration-time profile ( AUC ) ( BDCRB ) and AUC ( prodrug ) after l-Asp-BDCRB administration was roughly 3-fold greater than AUC ( BDCRB ) after BDCRB administration , suggesting that a reservoir of prodrug was delivered in addition to parent drug .
	manualset3
243982	8	422134	7	NULL	NULL	0	NULL	AUC	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the sum of area under the concentration-time profile ( AUC ) ( BDCRB ) and AUC ( prodrug ) after l-Asp-BDCRB administration was roughly 3-fold greater than AUC ( BDCRB ) after BDCRB administration , suggesting that a reservoir of prodrug was delivered in addition to parent drug .
	manualset3
243983	9	422134	7	NULL	NULL	0	NULL	BDCRB	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the sum of area under the concentration-time profile ( AUC ) ( BDCRB ) and AUC ( prodrug ) after l-Asp-BDCRB administration was roughly 3-fold greater than AUC ( BDCRB ) after BDCRB administration , suggesting that a reservoir of prodrug was delivered in addition to parent drug .
	manualset3
243984	10	422134	7	NULL	NULL	0	NULL	BDCRB administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the sum of area under the concentration-time profile ( AUC ) ( BDCRB ) and AUC ( prodrug ) after l-Asp-BDCRB administration was roughly 3-fold greater than AUC ( BDCRB ) after BDCRB administration , suggesting that a reservoir of prodrug was delivered in addition to parent drug .
	manualset3
243985	11	422134	7	NULL	NULL	0	NULL	reservoir	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the sum of area under the concentration-time profile ( AUC ) ( BDCRB ) and AUC ( prodrug ) after l-Asp-BDCRB administration was roughly 3-fold greater than AUC ( BDCRB ) after BDCRB administration , suggesting that a reservoir of prodrug was delivered in addition to parent drug .
	manualset3
243986	12	422134	7	NULL	NULL	0	NULL	prodrug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the sum of area under the concentration-time profile ( AUC ) ( BDCRB ) and AUC ( prodrug ) after l-Asp-BDCRB administration was roughly 3-fold greater than AUC ( BDCRB ) after BDCRB administration , suggesting that a reservoir of prodrug was delivered in addition to parent drug .
	manualset3
243987	13	422134	7	NULL	NULL	0	NULL	 parent drug 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Furthermore , the sum of area under the concentration-time profile ( AUC ) ( BDCRB ) and AUC ( prodrug ) after l-Asp-BDCRB administration was roughly 3-fold greater than AUC ( BDCRB ) after BDCRB administration , suggesting that a reservoir of prodrug was delivered in addition to parent drug .
	manualset3
243988	1	422135	7	NULL	NULL	0	NULL	score	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We were able to show that this score allowed to make the diagnosis of irritable bowel syndrome with accuracy because the specificity was 97 percent and the sensitivity was 83 percent .
	manualset3
243989	2	422135	7	NULL	NULL	0	NULL	diagnosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We were able to show that this score allowed to make the diagnosis of irritable bowel syndrome with accuracy because the specificity was 97 percent and the sensitivity was 83 percent .
	manualset3
243990	3	422135	7	NULL	NULL	0	NULL	 irritable bowel syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We were able to show that this score allowed to make the diagnosis of irritable bowel syndrome with accuracy because the specificity was 97 percent and the sensitivity was 83 percent .
	manualset3
243991	5	422135	7	NULL	NULL	NULL	NULL	97 percent 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We were able to show that this score allowed to make the diagnosis of irritable bowel syndrome with accuracy because the specificity was 97 percent and the sensitivity was 83 percent .
	manualset3
243992	4	422135	7	NULL	NULL	NULL	NULL	specificity	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We were able to show that this score allowed to make the diagnosis of irritable bowel syndrome with accuracy because the specificity was 97 percent and the sensitivity was 83 percent .
	manualset3
243993	6	422135	7	NULL	NULL	0	NULL	 sensitivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We were able to show that this score allowed to make the diagnosis of irritable bowel syndrome with accuracy because the specificity was 97 percent and the sensitivity was 83 percent .
	manualset3
243994	7	422135	7	NULL	NULL	0	NULL	83 percent 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We were able to show that this score allowed to make the diagnosis of irritable bowel syndrome with accuracy because the specificity was 97 percent and the sensitivity was 83 percent .
	manualset3
243995	1	422136	7	NULL	NULL	0	NULL	examination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An examination of the time course of responding revealed that the initial effect of clonidine was to decrease responses with the duration and magnitude of the decrease directly proportional to dose .
	manualset3
243996	2	422136	7	NULL	NULL	0	NULL	time course	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	An examination of the time course of responding revealed that the initial effect of clonidine was to decrease responses with the duration and magnitude of the decrease directly proportional to dose .
	manualset3
243997	3	422136	7	NULL	NULL	0	NULL	initial effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An examination of the time course of responding revealed that the initial effect of clonidine was to decrease responses with the duration and magnitude of the decrease directly proportional to dose .
	manualset3
243998	4	422136	7	NULL	NULL	0	NULL	clonidine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An examination of the time course of responding revealed that the initial effect of clonidine was to decrease responses with the duration and magnitude of the decrease directly proportional to dose .
	manualset3
243999	5	422136	7	NULL	NULL	0	NULL	responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An examination of the time course of responding revealed that the initial effect of clonidine was to decrease responses with the duration and magnitude of the decrease directly proportional to dose .
	manualset3
244000	6	422136	7	NULL	NULL	0	NULL	duration 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	An examination of the time course of responding revealed that the initial effect of clonidine was to decrease responses with the duration and magnitude of the decrease directly proportional to dose .
	manualset3
244001	7	422136	7	NULL	NULL	0	NULL	 magnitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An examination of the time course of responding revealed that the initial effect of clonidine was to decrease responses with the duration and magnitude of the decrease directly proportional to dose .
	manualset3
244002	8	422136	7	NULL	NULL	0	NULL	dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An examination of the time course of responding revealed that the initial effect of clonidine was to decrease responses with the duration and magnitude of the decrease directly proportional to dose .
	manualset3
245781	9	422136	7	NULL	NULL	0	NULL	decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An examination of the time course of responding revealed that the initial effect of clonidine was to decrease responses with the duration and magnitude of the decrease directly proportional to dose .
	manualset3
244003	1	422137	7	NULL	NULL	0	NULL	 SDS-PAGE	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , SDS-PAGE of whole-cell proteins could be used as a rapid and simple method for the discrimination of thermophilic bacteria as the first step of species identification .
	manualset3
244004	2	422137	7	NULL	NULL	0	NULL	whole-cell proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , SDS-PAGE of whole-cell proteins could be used as a rapid and simple method for the discrimination of thermophilic bacteria as the first step of species identification .
	manualset3
244005	3	422137	7	NULL	NULL	0	NULL	simple method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , SDS-PAGE of whole-cell proteins could be used as a rapid and simple method for the discrimination of thermophilic bacteria as the first step of species identification .
	manualset3
244006	4	422137	7	NULL	NULL	0	NULL	discrimination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , SDS-PAGE of whole-cell proteins could be used as a rapid and simple method for the discrimination of thermophilic bacteria as the first step of species identification .
	manualset3
244007	5	422137	7	NULL	NULL	0	NULL	thermophilic bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , SDS-PAGE of whole-cell proteins could be used as a rapid and simple method for the discrimination of thermophilic bacteria as the first step of species identification .
	manualset3
244008	6	422137	7	NULL	NULL	0	NULL	first step	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , SDS-PAGE of whole-cell proteins could be used as a rapid and simple method for the discrimination of thermophilic bacteria as the first step of species identification .
	manualset3
244009	7	422137	7	NULL	NULL	0	NULL	species identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , SDS-PAGE of whole-cell proteins could be used as a rapid and simple method for the discrimination of thermophilic bacteria as the first step of species identification .
	manualset3
244010	1	422138	7	NULL	NULL	0	NULL	Afferent pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Afferent and efferent pathways originating from the same cortical columns were studied by injecting a mixture of PHA-L and wheat germ agglutinin conjugated to horseradish peroxidase ( WGA-HRP ) .
	manualset3
244011	2	422138	7	NULL	NULL	0	NULL	efferent pathways 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Afferent and efferent pathways originating from the same cortical columns were studied by injecting a mixture of PHA-L and wheat germ agglutinin conjugated to horseradish peroxidase ( WGA-HRP ) .
	manualset3
244012	3	422138	7	NULL	NULL	0	NULL	cortical columns 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Afferent and efferent pathways originating from the same cortical columns were studied by injecting a mixture of PHA-L and wheat germ agglutinin conjugated to horseradish peroxidase ( WGA-HRP ) .
	manualset3
244013	4	422138	7	NULL	NULL	0	NULL	mixture 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Afferent and efferent pathways originating from the same cortical columns were studied by injecting a mixture of PHA-L and wheat germ agglutinin conjugated to horseradish peroxidase ( WGA-HRP ) .
	manualset3
244014	5	422138	7	NULL	NULL	0	NULL	PHA-L	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Afferent and efferent pathways originating from the same cortical columns were studied by injecting a mixture of PHA-L and wheat germ agglutinin conjugated to horseradish peroxidase ( WGA-HRP ) .
	manualset3
244015	6	422138	7	NULL	NULL	0	NULL	 wheat germ agglutinin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Afferent and efferent pathways originating from the same cortical columns were studied by injecting a mixture of PHA-L and wheat germ agglutinin conjugated to horseradish peroxidase ( WGA-HRP ) .
	manualset3
244016	7	422138	7	NULL	NULL	0	NULL	horseradish peroxidase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Afferent and efferent pathways originating from the same cortical columns were studied by injecting a mixture of PHA-L and wheat germ agglutinin conjugated to horseradish peroxidase ( WGA-HRP ) .
	manualset3
244017	8	422138	7	NULL	NULL	0	NULL	WGA-HRP	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Afferent and efferent pathways originating from the same cortical columns were studied by injecting a mixture of PHA-L and wheat germ agglutinin conjugated to horseradish peroxidase ( WGA-HRP ) .
	manualset3
244018	1	422139	7	NULL	NULL	0	NULL	 potential immunotherapeutic efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we examined the potential immunotherapeutic efficacy of the subunit vaccine Leish-111f + MPL-SE , which has undergone rigorous preclinical testing and been demonstrated safe in human clinical trials .
	manualset3
244019	2	422139	7	NULL	NULL	0	NULL	subunit vaccine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we examined the potential immunotherapeutic efficacy of the subunit vaccine Leish-111f + MPL-SE , which has undergone rigorous preclinical testing and been demonstrated safe in human clinical trials .
	manualset3
244020	3	422139	7	NULL	NULL	0	NULL	Leish-111f + MPL-SE	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we examined the potential immunotherapeutic efficacy of the subunit vaccine Leish-111f + MPL-SE , which has undergone rigorous preclinical testing and been demonstrated safe in human clinical trials .
	manualset3
244021	4	422139	7	NULL	NULL	0	NULL	preclinical testing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we examined the potential immunotherapeutic efficacy of the subunit vaccine Leish-111f + MPL-SE , which has undergone rigorous preclinical testing and been demonstrated safe in human clinical trials .
	manualset3
244022	5	422139	7	NULL	NULL	0	NULL	 human clinical trials	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Therefore , we examined the potential immunotherapeutic efficacy of the subunit vaccine Leish-111f + MPL-SE , which has undergone rigorous preclinical testing and been demonstrated safe in human clinical trials .
	manualset3
244023	1	422140	7	NULL	NULL	0	NULL	Binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Binding of antibodies against birch pollen antigens/allergens to various parts of apples as studied by immuno-gold electron microscopy .
	manualset3
244024	2	422140	7	NULL	NULL	0	NULL	antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Binding of antibodies against birch pollen antigens/allergens to various parts of apples as studied by immuno-gold electron microscopy .
	manualset3
244025	3	422140	7	NULL	NULL	0	NULL	birch pollen antigens	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Binding of antibodies against birch pollen antigens/allergens to various parts of apples as studied by immuno-gold electron microscopy .
	manualset3
244026	4	422140	7	NULL	NULL	0	NULL	allergens 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Binding of antibodies against birch pollen antigens/allergens to various parts of apples as studied by immuno-gold electron microscopy .
	manualset3
244027	5	422140	7	NULL	NULL	0	NULL	apples	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Binding of antibodies against birch pollen antigens/allergens to various parts of apples as studied by immuno-gold electron microscopy .
	manualset3
244028	6	422140	7	NULL	NULL	0	NULL	immuno-gold electron microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Binding of antibodies against birch pollen antigens/allergens to various parts of apples as studied by immuno-gold electron microscopy .
	manualset3
244029	1	422141	7	NULL	NULL	0	NULL	Hypophosphatasia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypophosphatasia is a rare disease characterized by low serum levels of tissue non-specific alkaline phosphatase ( TNSALP ) and a spectrum of skeletal disease varying from the severest form with death in utero to mild with no clinical abnormality in adults .
	manualset3
244030	2	422141	7	NULL	NULL	0	NULL	rare disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypophosphatasia is a rare disease characterized by low serum levels of tissue non-specific alkaline phosphatase ( TNSALP ) and a spectrum of skeletal disease varying from the severest form with death in utero to mild with no clinical abnormality in adults .
	manualset3
244031	3	422141	7	NULL	NULL	0	NULL	low serum levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypophosphatasia is a rare disease characterized by low serum levels of tissue non-specific alkaline phosphatase ( TNSALP ) and a spectrum of skeletal disease varying from the severest form with death in utero to mild with no clinical abnormality in adults .
	manualset3
244032	4	422141	7	NULL	NULL	0	NULL	tissue non-specific alkaline phosphatase ( TNSALP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypophosphatasia is a rare disease characterized by low serum levels of tissue non-specific alkaline phosphatase ( TNSALP ) and a spectrum of skeletal disease varying from the severest form with death in utero to mild with no clinical abnormality in adults .
	manualset3
244033	5	422141	7	NULL	NULL	0	NULL	spectrum	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypophosphatasia is a rare disease characterized by low serum levels of tissue non-specific alkaline phosphatase ( TNSALP ) and a spectrum of skeletal disease varying from the severest form with death in utero to mild with no clinical abnormality in adults .
	manualset3
244034	6	422141	7	NULL	NULL	0	NULL	skeletal disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypophosphatasia is a rare disease characterized by low serum levels of tissue non-specific alkaline phosphatase ( TNSALP ) and a spectrum of skeletal disease varying from the severest form with death in utero to mild with no clinical abnormality in adults .
	manualset3
244035	7	422141	7	NULL	NULL	0	NULL	severest form	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypophosphatasia is a rare disease characterized by low serum levels of tissue non-specific alkaline phosphatase ( TNSALP ) and a spectrum of skeletal disease varying from the severest form with death in utero to mild with no clinical abnormality in adults .
	manualset3
244036	8	422141	7	NULL	NULL	0	NULL	death 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypophosphatasia is a rare disease characterized by low serum levels of tissue non-specific alkaline phosphatase ( TNSALP ) and a spectrum of skeletal disease varying from the severest form with death in utero to mild with no clinical abnormality in adults .
	manualset3
244037	9	422141	7	NULL	NULL	0	NULL	 clinical abnormality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypophosphatasia is a rare disease characterized by low serum levels of tissue non-specific alkaline phosphatase ( TNSALP ) and a spectrum of skeletal disease varying from the severest form with death in utero to mild with no clinical abnormality in adults .
	manualset3
244038	10	422141	7	NULL	NULL	0	NULL	adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypophosphatasia is a rare disease characterized by low serum levels of tissue non-specific alkaline phosphatase ( TNSALP ) and a spectrum of skeletal disease varying from the severest form with death in utero to mild with no clinical abnormality in adults .
	manualset3
244039	1	422142	7	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on stability of aneurine in solution in presence of ascorbic acid and cysteine ) .
	manualset3
244040	2	422142	7	NULL	NULL	0	NULL	stability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on stability of aneurine in solution in presence of ascorbic acid and cysteine ) .
	manualset3
244041	3	422142	7	NULL	NULL	0	NULL	aneurine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on stability of aneurine in solution in presence of ascorbic acid and cysteine ) .
	manualset3
244042	4	422142	7	NULL	NULL	0	NULL	solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on stability of aneurine in solution in presence of ascorbic acid and cysteine ) .
	manualset3
244043	5	422142	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on stability of aneurine in solution in presence of ascorbic acid and cysteine ) .
	manualset3
244044	6	422142	7	NULL	NULL	0	NULL	ascorbic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on stability of aneurine in solution in presence of ascorbic acid and cysteine ) .
	manualset3
244045	7	422142	7	NULL	NULL	0	NULL	cysteine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	( Studies on stability of aneurine in solution in presence of ascorbic acid and cysteine ) .
	manualset3
244083	1	422143	7	NULL	NULL	0	NULL	Diagnostic quiz	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Diagnostic quiz : Orange-colored urine ) .
	manualset3
244084	2	422143	7	NULL	NULL	0	NULL	Orange-colored urine 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Diagnostic quiz : Orange-colored urine ) .
	manualset3
244085	1	422144	7	NULL	NULL	0	NULL	example	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An example is presented , which highlights the importance of the sampling step in the quality of analytical results .
	manualset3
244086	2	422144	7	NULL	NULL	NULL	NULL	sampling step	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An example is presented , which highlights the importance of the sampling step in the quality of analytical results .
	manualset3
244087	3	422144	7	NULL	NULL	0	NULL	quality	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An example is presented , which highlights the importance of the sampling step in the quality of analytical results .
	manualset3
244088	4	422144	7	NULL	NULL	0	NULL	analytical results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An example is presented , which highlights the importance of the sampling step in the quality of analytical results .
	manualset3
244089	1	422145	7	NULL	NULL	0	NULL	 synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis , structural characterization and the study of the photophysical properties of complexes ( AuCu ( C6F5 ) 2 ( N ( triple bond ) C-CH3 ) 2 ) 1 , ( AuCu ( C6F5 ) 2 ( N ( triple bond ) C-Ph ) 2 ) 2 2 , and ( AuCu ( C6F5 ) 2 ( N ( triple bond ) C-CH = CH-Ph ) 2 ) 3 have been carried out .
	manualset3
244090	2	422145	7	NULL	NULL	0	NULL	structural characterization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis , structural characterization and the study of the photophysical properties of complexes ( AuCu ( C6F5 ) 2 ( N ( triple bond ) C-CH3 ) 2 ) 1 , ( AuCu ( C6F5 ) 2 ( N ( triple bond ) C-Ph ) 2 ) 2 2 , and ( AuCu ( C6F5 ) 2 ( N ( triple bond ) C-CH = CH-Ph ) 2 ) 3 have been carried out .
	manualset3
244091	3	422145	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis , structural characterization and the study of the photophysical properties of complexes ( AuCu ( C6F5 ) 2 ( N ( triple bond ) C-CH3 ) 2 ) 1 , ( AuCu ( C6F5 ) 2 ( N ( triple bond ) C-Ph ) 2 ) 2 2 , and ( AuCu ( C6F5 ) 2 ( N ( triple bond ) C-CH = CH-Ph ) 2 ) 3 have been carried out .
	manualset3
244092	4	422145	7	NULL	NULL	0	NULL	photophysical properties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis , structural characterization and the study of the photophysical properties of complexes ( AuCu ( C6F5 ) 2 ( N ( triple bond ) C-CH3 ) 2 ) 1 , ( AuCu ( C6F5 ) 2 ( N ( triple bond ) C-Ph ) 2 ) 2 2 , and ( AuCu ( C6F5 ) 2 ( N ( triple bond ) C-CH = CH-Ph ) 2 ) 3 have been carried out .
	manualset3
244093	5	422145	7	NULL	NULL	0	NULL	complexes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis , structural characterization and the study of the photophysical properties of complexes ( AuCu ( C6F5 ) 2 ( N ( triple bond ) C-CH3 ) 2 ) 1 , ( AuCu ( C6F5 ) 2 ( N ( triple bond ) C-Ph ) 2 ) 2 2 , and ( AuCu ( C6F5 ) 2 ( N ( triple bond ) C-CH = CH-Ph ) 2 ) 3 have been carried out .
	manualset3
244094	6	422145	7	NULL	NULL	0	NULL	 ( AuCu ( C6F5 ) 2 ( N ( triple bond ) C-CH3 ) 2 ) 1	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis , structural characterization and the study of the photophysical properties of complexes ( AuCu ( C6F5 ) 2 ( N ( triple bond ) C-CH3 ) 2 ) 1 , ( AuCu ( C6F5 ) 2 ( N ( triple bond ) C-Ph ) 2 ) 2 2 , and ( AuCu ( C6F5 ) 2 ( N ( triple bond ) C-CH = CH-Ph ) 2 ) 3 have been carried out .
	manualset3
244095	7	422145	7	NULL	NULL	0	NULL	( AuCu ( C6F5 ) 2 ( N ( triple bond ) C-Ph ) 2 ) 2 2 ,	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis , structural characterization and the study of the photophysical properties of complexes ( AuCu ( C6F5 ) 2 ( N ( triple bond ) C-CH3 ) 2 ) 1 , ( AuCu ( C6F5 ) 2 ( N ( triple bond ) C-Ph ) 2 ) 2 2 , and ( AuCu ( C6F5 ) 2 ( N ( triple bond ) C-CH = CH-Ph ) 2 ) 3 have been carried out .
	manualset3
244096	8	422145	7	NULL	NULL	0	NULL	( AuCu ( C6F5 ) 2 ( N ( triple bond ) C-CH = CH-Ph ) 2 ) 3 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The synthesis , structural characterization and the study of the photophysical properties of complexes ( AuCu ( C6F5 ) 2 ( N ( triple bond ) C-CH3 ) 2 ) 1 , ( AuCu ( C6F5 ) 2 ( N ( triple bond ) C-Ph ) 2 ) 2 2 , and ( AuCu ( C6F5 ) 2 ( N ( triple bond ) C-CH = CH-Ph ) 2 ) 3 have been carried out .
	manualset3
244097	1	422146	7	NULL	NULL	NULL	NULL	Disseminated effects	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Disseminated effects on the central nervous system were similar to those of adults with multiple sclerosis .
	manualset3
244098	2	422146	7	NULL	NULL	0	NULL	central nervous system 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Disseminated effects on the central nervous system were similar to those of adults with multiple sclerosis .
	manualset3
244099	3	422146	7	NULL	NULL	0	NULL	adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Disseminated effects on the central nervous system were similar to those of adults with multiple sclerosis .
	manualset3
244100	4	422146	7	NULL	NULL	0	NULL	multiple sclerosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Disseminated effects on the central nervous system were similar to those of adults with multiple sclerosis .
	manualset3
244101	1	422147	7	NULL	NULL	0	NULL	mechanoreceptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Resembling mechanoreceptors cytologically , the spinal CSF-contacting neurons send their axons to the outer surface of the spinal cord to form neurosecretory-type terminals .
	manualset3
244102	2	422147	7	NULL	NULL	0	NULL	spinal CSF-contacting neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Resembling mechanoreceptors cytologically , the spinal CSF-contacting neurons send their axons to the outer surface of the spinal cord to form neurosecretory-type terminals .
	manualset3
244103	3	422147	7	NULL	NULL	0	NULL	axons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Resembling mechanoreceptors cytologically , the spinal CSF-contacting neurons send their axons to the outer surface of the spinal cord to form neurosecretory-type terminals .
	manualset3
244104	4	422147	7	NULL	NULL	0	NULL	outer surface	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Resembling mechanoreceptors cytologically , the spinal CSF-contacting neurons send their axons to the outer surface of the spinal cord to form neurosecretory-type terminals .
	manualset3
244105	5	422147	7	NULL	NULL	0	NULL	 spinal cord 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Resembling mechanoreceptors cytologically , the spinal CSF-contacting neurons send their axons to the outer surface of the spinal cord to form neurosecretory-type terminals .
	manualset3
244106	6	422147	7	NULL	NULL	0	NULL	neurosecretory-type terminals	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Resembling mechanoreceptors cytologically , the spinal CSF-contacting neurons send their axons to the outer surface of the spinal cord to form neurosecretory-type terminals .
	manualset3
244107	1	422148	7	NULL	NULL	0	NULL	 mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This indeed may be the mechanism of action of central sympatholytic antihypertensives such as alpha-methyldopa .
	manualset3
244108	2	422148	7	NULL	NULL	0	NULL	 action 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This indeed may be the mechanism of action of central sympatholytic antihypertensives such as alpha-methyldopa .
	manualset3
244109	3	422148	7	NULL	NULL	0	NULL	central sympatholytic antihypertensives	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	This indeed may be the mechanism of action of central sympatholytic antihypertensives such as alpha-methyldopa .
	manualset3
244110	4	422148	7	NULL	NULL	0	NULL	alpha-methyldopa	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	This indeed may be the mechanism of action of central sympatholytic antihypertensives such as alpha-methyldopa .
	manualset3
244111	1	422149	7	NULL	NULL	0	NULL	thymus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	It is possible that the thymus is involved in the origin of immunopathological reactions and a target during malaria infections .
	manualset3
244112	2	422149	7	NULL	NULL	NULL	NULL	 origin 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is possible that the thymus is involved in the origin of immunopathological reactions and a target during malaria infections .
	manualset3
244113	3	422149	7	NULL	NULL	0	NULL	immunopathological reactions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It is possible that the thymus is involved in the origin of immunopathological reactions and a target during malaria infections .
	manualset3
244114	4	422149	7	NULL	NULL	0	NULL	malaria infections	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	It is possible that the thymus is involved in the origin of immunopathological reactions and a target during malaria infections .
	manualset3
245782	5	422149	7	NULL	NULL	NULL	NULL	target	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	It is possible that the thymus is involved in the origin of immunopathological reactions and a target during malaria infections .
	manualset3
244115	1	422150	7	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	An excellent correlation was observed between the IF and biochemical methods when specimens contained greater than 5 % TdT + cells ( by IF ) ; below this level the biochemical assay was less reliable , while the sensitive IF test could detect isolated TdT + cells among greater than 10 000 TdT negative cells .
	manualset3
244116	2	422150	7	NULL	NULL	0	NULL	IF	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An excellent correlation was observed between the IF and biochemical methods when specimens contained greater than 5 % TdT + cells ( by IF ) ; below this level the biochemical assay was less reliable , while the sensitive IF test could detect isolated TdT + cells among greater than 10 000 TdT negative cells .
	manualset3
244117	3	422150	7	NULL	NULL	0	NULL	biochemical methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An excellent correlation was observed between the IF and biochemical methods when specimens contained greater than 5 % TdT + cells ( by IF ) ; below this level the biochemical assay was less reliable , while the sensitive IF test could detect isolated TdT + cells among greater than 10 000 TdT negative cells .
	manualset3
244118	4	422150	7	NULL	NULL	0	NULL	specimens	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	An excellent correlation was observed between the IF and biochemical methods when specimens contained greater than 5 % TdT + cells ( by IF ) ; below this level the biochemical assay was less reliable , while the sensitive IF test could detect isolated TdT + cells among greater than 10 000 TdT negative cells .
	manualset3
244119	5	422150	7	NULL	NULL	0	NULL	5 % TdT + cells 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An excellent correlation was observed between the IF and biochemical methods when specimens contained greater than 5 % TdT + cells ( by IF ) ; below this level the biochemical assay was less reliable , while the sensitive IF test could detect isolated TdT + cells among greater than 10 000 TdT negative cells .
	manualset3
244120	6	422150	7	NULL	NULL	0	NULL	IF	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An excellent correlation was observed between the IF and biochemical methods when specimens contained greater than 5 % TdT + cells ( by IF ) ; below this level the biochemical assay was less reliable , while the sensitive IF test could detect isolated TdT + cells among greater than 10 000 TdT negative cells .
	manualset3
244121	7	422150	7	NULL	NULL	0	NULL	level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An excellent correlation was observed between the IF and biochemical methods when specimens contained greater than 5 % TdT + cells ( by IF ) ; below this level the biochemical assay was less reliable , while the sensitive IF test could detect isolated TdT + cells among greater than 10 000 TdT negative cells .
	manualset3
244122	8	422150	7	NULL	NULL	0	NULL	biochemical assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An excellent correlation was observed between the IF and biochemical methods when specimens contained greater than 5 % TdT + cells ( by IF ) ; below this level the biochemical assay was less reliable , while the sensitive IF test could detect isolated TdT + cells among greater than 10 000 TdT negative cells .
	manualset3
244123	9	422150	7	NULL	NULL	0	NULL	sensitive IF test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An excellent correlation was observed between the IF and biochemical methods when specimens contained greater than 5 % TdT + cells ( by IF ) ; below this level the biochemical assay was less reliable , while the sensitive IF test could detect isolated TdT + cells among greater than 10 000 TdT negative cells .
	manualset3
244124	10	422150	7	NULL	NULL	0	NULL	isolated TdT + cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	An excellent correlation was observed between the IF and biochemical methods when specimens contained greater than 5 % TdT + cells ( by IF ) ; below this level the biochemical assay was less reliable , while the sensitive IF test could detect isolated TdT + cells among greater than 10 000 TdT negative cells .
	manualset3
244125	11	422150	7	NULL	NULL	0	NULL	10 000 TdT negative cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	An excellent correlation was observed between the IF and biochemical methods when specimens contained greater than 5 % TdT + cells ( by IF ) ; below this level the biochemical assay was less reliable , while the sensitive IF test could detect isolated TdT + cells among greater than 10 000 TdT negative cells .
	manualset3
244126	1	422151	7	NULL	NULL	0	NULL	Transformation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Transformation and degradation of sugars in diluted strong acid solution ) .
	manualset3
244127	2	422151	7	NULL	NULL	0	NULL	 degradation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Transformation and degradation of sugars in diluted strong acid solution ) .
	manualset3
244128	3	422151	7	NULL	NULL	0	NULL	sugars	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Transformation and degradation of sugars in diluted strong acid solution ) .
	manualset3
244129	4	422151	7	NULL	NULL	0	NULL	diluted strong acid solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	I. Transformation and degradation of sugars in diluted strong acid solution ) .
	manualset3
244130	1	422152	7	NULL	NULL	0	NULL	rhythm	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the perceived advantages of rhythm were that it permits spontaneous intercourse on the safe days and has no bad side effects .
	manualset3
244131	2	422152	7	NULL	NULL	0	NULL	 spontaneous intercourse	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the perceived advantages of rhythm were that it permits spontaneous intercourse on the safe days and has no bad side effects .
	manualset3
244132	3	422152	7	NULL	NULL	0	NULL	safe days	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the perceived advantages of rhythm were that it permits spontaneous intercourse on the safe days and has no bad side effects .
	manualset3
244133	4	422152	7	NULL	NULL	0	NULL	no bad side effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the perceived advantages of rhythm were that it permits spontaneous intercourse on the safe days and has no bad side effects .
	manualset3
244134	5	422152	7	NULL	NULL	0	NULL	advantages	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Among the perceived advantages of rhythm were that it permits spontaneous intercourse on the safe days and has no bad side effects .
	manualset3
244135	1	422153	7	NULL	NULL	0	NULL	Selective removal 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective removal of alloreactive cells from hematopoietic stem cell grafts : graft engineering for GVHD prophylaxis .
	manualset3
244136	2	422153	7	NULL	NULL	0	NULL	alloreactive cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective removal of alloreactive cells from hematopoietic stem cell grafts : graft engineering for GVHD prophylaxis .
	manualset3
244137	3	422153	7	NULL	NULL	0	NULL	 hematopoietic stem cell grafts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective removal of alloreactive cells from hematopoietic stem cell grafts : graft engineering for GVHD prophylaxis .
	manualset3
244138	4	422153	7	NULL	NULL	0	NULL	 graft engineering	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective removal of alloreactive cells from hematopoietic stem cell grafts : graft engineering for GVHD prophylaxis .
	manualset3
244139	5	422153	7	NULL	NULL	0	NULL	GVHD prophylaxis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Selective removal of alloreactive cells from hematopoietic stem cell grafts : graft engineering for GVHD prophylaxis .
	manualset3
244140	1	422154	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( The use of epsilon-aminocaproic acid in prostatic surgery ) .
	manualset3
244141	2	422154	7	NULL	NULL	0	NULL	epsilon-aminocaproic acid 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( The use of epsilon-aminocaproic acid in prostatic surgery ) .
	manualset3
244142	3	422154	7	NULL	NULL	0	NULL	prostatic surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( The use of epsilon-aminocaproic acid in prostatic surgery ) .
	manualset3
244143	1	422155	7	NULL	NULL	0	NULL	Neurology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Neurology , neuropsychology and neurosciences : on the use and abuse of the term neuro ) .
	manualset3
244144	2	422155	7	NULL	NULL	0	NULL	neuropsychology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Neurology , neuropsychology and neurosciences : on the use and abuse of the term neuro ) .
	manualset3
244145	3	422155	7	NULL	NULL	0	NULL	neurosciences	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Neurology , neuropsychology and neurosciences : on the use and abuse of the term neuro ) .
	manualset3
244146	4	422155	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Neurology , neuropsychology and neurosciences : on the use and abuse of the term neuro ) .
	manualset3
244147	5	422155	7	NULL	NULL	0	NULL	neuro 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Neurology , neuropsychology and neurosciences : on the use and abuse of the term neuro ) .
	manualset3
244161	1	422156	7	NULL	NULL	0	NULL	abundance	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The abundance of BP-3 mRNA was dramatically lowered by ( Bu ) 2cAMP , but was unaffected by IGF-I .
	manualset3
244162	2	422156	7	NULL	NULL	0	NULL	BP-3 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The abundance of BP-3 mRNA was dramatically lowered by ( Bu ) 2cAMP , but was unaffected by IGF-I .
	manualset3
244163	3	422156	7	NULL	NULL	0	NULL	( Bu ) 2cAMP 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The abundance of BP-3 mRNA was dramatically lowered by ( Bu ) 2cAMP , but was unaffected by IGF-I .
	manualset3
244164	4	422156	7	NULL	NULL	0	NULL	IGF-I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The abundance of BP-3 mRNA was dramatically lowered by ( Bu ) 2cAMP , but was unaffected by IGF-I .
	manualset3
244165	1	422157	7	NULL	NULL	0	NULL	column	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	On a column of entrapped phospholipid-stearylamine ( 4 : 1 ) ( cationic ) vesicles , 0.36 mg of ferritin was bound per mumol lipids at 0.05 M ionic strength and pH 7 .
	manualset3
244166	2	422157	7	NULL	NULL	0	NULL	phospholipid-stearylamine ( 4 : 1 ) ( cationic ) vesicles 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	On a column of entrapped phospholipid-stearylamine ( 4 : 1 ) ( cationic ) vesicles , 0.36 mg of ferritin was bound per mumol lipids at 0.05 M ionic strength and pH 7 .
	manualset3
244167	3	422157	7	NULL	NULL	0	NULL	0.36 mg	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On a column of entrapped phospholipid-stearylamine ( 4 : 1 ) ( cationic ) vesicles , 0.36 mg of ferritin was bound per mumol lipids at 0.05 M ionic strength and pH 7 .
	manualset3
244168	4	422157	7	NULL	NULL	0	NULL	ferritin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	On a column of entrapped phospholipid-stearylamine ( 4 : 1 ) ( cationic ) vesicles , 0.36 mg of ferritin was bound per mumol lipids at 0.05 M ionic strength and pH 7 .
	manualset3
244169	5	422157	7	NULL	NULL	0	NULL	 per mumol lipids	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On a column of entrapped phospholipid-stearylamine ( 4 : 1 ) ( cationic ) vesicles , 0.36 mg of ferritin was bound per mumol lipids at 0.05 M ionic strength and pH 7 .
	manualset3
244170	6	422157	7	NULL	NULL	0	NULL	0.05 M ionic strength	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On a column of entrapped phospholipid-stearylamine ( 4 : 1 ) ( cationic ) vesicles , 0.36 mg of ferritin was bound per mumol lipids at 0.05 M ionic strength and pH 7 .
	manualset3
244171	7	422157	7	NULL	NULL	0	NULL	pH 7	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On a column of entrapped phospholipid-stearylamine ( 4 : 1 ) ( cationic ) vesicles , 0.36 mg of ferritin was bound per mumol lipids at 0.05 M ionic strength and pH 7 .
	manualset3
244172	1	422158	7	NULL	NULL	0	NULL	 frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of self-reference statements as a function of generalized reinforcement .
	manualset3
244173	2	422158	7	NULL	NULL	0	NULL	self-reference statements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of self-reference statements as a function of generalized reinforcement .
	manualset3
244174	3	422158	7	NULL	NULL	0	NULL	function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of self-reference statements as a function of generalized reinforcement .
	manualset3
244175	4	422158	7	NULL	NULL	0	NULL	generalized reinforcement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The frequency of self-reference statements as a function of generalized reinforcement .
	manualset3
244176	1	422159	7	NULL	NULL	0	NULL	Two-parameter sorting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-parameter sorting based on DNA and light scatter indicated that slowly cycling cells were larger than the average .
	manualset3
244177	2	422159	7	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-parameter sorting based on DNA and light scatter indicated that slowly cycling cells were larger than the average .
	manualset3
244178	3	422159	7	NULL	NULL	0	NULL	light scatter	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-parameter sorting based on DNA and light scatter indicated that slowly cycling cells were larger than the average .
	manualset3
244179	4	422159	7	NULL	NULL	0	NULL	slowly cycling cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-parameter sorting based on DNA and light scatter indicated that slowly cycling cells were larger than the average .
	manualset3
244180	5	422159	7	NULL	NULL	0	NULL	average 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-parameter sorting based on DNA and light scatter indicated that slowly cycling cells were larger than the average .
	manualset3
244181	1	422160	7	NULL	NULL	0	NULL	akathisia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The akathisia experienced after administration of the test of haloperidol dose was not mild or inconsequential ; 28 % of the patients experienced moderate , 17 % of the patients experienced severe , and 22 % of the patients experienced very severe akathisia .
	manualset3
244182	2	422160	7	NULL	NULL	0	NULL	administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The akathisia experienced after administration of the test of haloperidol dose was not mild or inconsequential ; 28 % of the patients experienced moderate , 17 % of the patients experienced severe , and 22 % of the patients experienced very severe akathisia .
	manualset3
244183	3	422160	7	NULL	NULL	0	NULL	test	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The akathisia experienced after administration of the test of haloperidol dose was not mild or inconsequential ; 28 % of the patients experienced moderate , 17 % of the patients experienced severe , and 22 % of the patients experienced very severe akathisia .
	manualset3
244184	4	422160	7	NULL	NULL	0	NULL	haloperidol dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The akathisia experienced after administration of the test of haloperidol dose was not mild or inconsequential ; 28 % of the patients experienced moderate , 17 % of the patients experienced severe , and 22 % of the patients experienced very severe akathisia .
	manualset3
244185	5	422160	7	NULL	NULL	0	NULL	 28 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The akathisia experienced after administration of the test of haloperidol dose was not mild or inconsequential ; 28 % of the patients experienced moderate , 17 % of the patients experienced severe , and 22 % of the patients experienced very severe akathisia .
	manualset3
244186	6	422160	7	NULL	NULL	0	NULL	 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The akathisia experienced after administration of the test of haloperidol dose was not mild or inconsequential ; 28 % of the patients experienced moderate , 17 % of the patients experienced severe , and 22 % of the patients experienced very severe akathisia .
	manualset3
244187	7	422160	7	NULL	NULL	0	NULL	17 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The akathisia experienced after administration of the test of haloperidol dose was not mild or inconsequential ; 28 % of the patients experienced moderate , 17 % of the patients experienced severe , and 22 % of the patients experienced very severe akathisia .
	manualset3
244188	8	422160	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The akathisia experienced after administration of the test of haloperidol dose was not mild or inconsequential ; 28 % of the patients experienced moderate , 17 % of the patients experienced severe , and 22 % of the patients experienced very severe akathisia .
	manualset3
244189	9	422160	7	NULL	NULL	0	NULL	22 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The akathisia experienced after administration of the test of haloperidol dose was not mild or inconsequential ; 28 % of the patients experienced moderate , 17 % of the patients experienced severe , and 22 % of the patients experienced very severe akathisia .
	manualset3
244190	10	422160	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The akathisia experienced after administration of the test of haloperidol dose was not mild or inconsequential ; 28 % of the patients experienced moderate , 17 % of the patients experienced severe , and 22 % of the patients experienced very severe akathisia .
	manualset3
244191	11	422160	7	NULL	NULL	0	NULL	severe akathisia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The akathisia experienced after administration of the test of haloperidol dose was not mild or inconsequential ; 28 % of the patients experienced moderate , 17 % of the patients experienced severe , and 22 % of the patients experienced very severe akathisia .
	manualset3
244214	1	422161	7	NULL	NULL	0	NULL	Highly mechanised systems	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly mechanised systems , such as hydraulic tailgate lifts , are not recommended in developing countries due to maintenance difficulties .
	manualset3
244215	2	422161	7	NULL	NULL	0	NULL	hydraulic tailgate lifts	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly mechanised systems , such as hydraulic tailgate lifts , are not recommended in developing countries due to maintenance difficulties .
	manualset3
244216	3	422161	7	NULL	NULL	0	NULL	developing countries	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly mechanised systems , such as hydraulic tailgate lifts , are not recommended in developing countries due to maintenance difficulties .
	manualset3
244217	4	422161	7	NULL	NULL	0	NULL	difficulties	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Highly mechanised systems , such as hydraulic tailgate lifts , are not recommended in developing countries due to maintenance difficulties .
	manualset3
244219	1	422162	7	NULL	NULL	0	NULL	Forced migration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Forced migration and mortality in the very long term : did perestroika affect death rates also in Finland ?
	manualset3
244220	2	422162	7	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Forced migration and mortality in the very long term : did perestroika affect death rates also in Finland ?
	manualset3
244221	3	422162	7	NULL	NULL	0	NULL	long term	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Forced migration and mortality in the very long term : did perestroika affect death rates also in Finland ?
	manualset3
244223	4	422162	7	NULL	NULL	0	NULL	 perestroika	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Forced migration and mortality in the very long term : did perestroika affect death rates also in Finland ?
	manualset3
244225	5	422162	7	NULL	NULL	0	NULL	death rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Forced migration and mortality in the very long term : did perestroika affect death rates also in Finland ?
	manualset3
244226	6	422162	7	NULL	NULL	0	NULL	Finland	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Forced migration and mortality in the very long term : did perestroika affect death rates also in Finland ?
	manualset3
244228	1	422163	7	NULL	NULL	NULL	NULL	Allogeneic mixed lymphocyte reactions	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Allogeneic mixed lymphocyte reactions revealed similar antigen-presenting functions of untransduced and lentivirally transduced DCs .
	manualset3
244229	2	422163	7	NULL	NULL	0	NULL	antigen-presenting functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Allogeneic mixed lymphocyte reactions revealed similar antigen-presenting functions of untransduced and lentivirally transduced DCs .
	manualset3
244231	3	422163	7	NULL	NULL	0	NULL	untransduced DCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Allogeneic mixed lymphocyte reactions revealed similar antigen-presenting functions of untransduced and lentivirally transduced DCs .
	manualset3
244232	4	422163	7	NULL	NULL	0	NULL	lentivirally transduced DCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Allogeneic mixed lymphocyte reactions revealed similar antigen-presenting functions of untransduced and lentivirally transduced DCs .
	manualset3
244233	1	422164	7	NULL	NULL	0	NULL	monomer-dimer equilibrium constant	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The monomer-dimer equilibrium constant of the oxidized holoenzyme at 25 degrees C was estimated to be 7 X 10 ( 5 ) M-1 at pH 7.5 and 4X 10 ( 6 ) M-1 at pH 8.3 .
	manualset3
244234	2	422164	7	NULL	NULL	0	NULL	oxidized holoenzyme	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The monomer-dimer equilibrium constant of the oxidized holoenzyme at 25 degrees C was estimated to be 7 X 10 ( 5 ) M-1 at pH 7.5 and 4X 10 ( 6 ) M-1 at pH 8.3 .
	manualset3
244235	3	422164	7	NULL	NULL	0	NULL	25 degrees C	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The monomer-dimer equilibrium constant of the oxidized holoenzyme at 25 degrees C was estimated to be 7 X 10 ( 5 ) M-1 at pH 7.5 and 4X 10 ( 6 ) M-1 at pH 8.3 .
	manualset3
244236	4	422164	7	NULL	NULL	0	NULL	7 X 10 ( 5 ) M-1	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The monomer-dimer equilibrium constant of the oxidized holoenzyme at 25 degrees C was estimated to be 7 X 10 ( 5 ) M-1 at pH 7.5 and 4X 10 ( 6 ) M-1 at pH 8.3 .
	manualset3
244237	5	422164	7	NULL	NULL	0	NULL	pH 7.5	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The monomer-dimer equilibrium constant of the oxidized holoenzyme at 25 degrees C was estimated to be 7 X 10 ( 5 ) M-1 at pH 7.5 and 4X 10 ( 6 ) M-1 at pH 8.3 .
	manualset3
244238	6	422164	7	NULL	NULL	0	NULL	4X 10 ( 6 ) M-1	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The monomer-dimer equilibrium constant of the oxidized holoenzyme at 25 degrees C was estimated to be 7 X 10 ( 5 ) M-1 at pH 7.5 and 4X 10 ( 6 ) M-1 at pH 8.3 .
	manualset3
244239	7	422164	7	NULL	NULL	0	NULL	pH 8.3	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The monomer-dimer equilibrium constant of the oxidized holoenzyme at 25 degrees C was estimated to be 7 X 10 ( 5 ) M-1 at pH 7.5 and 4X 10 ( 6 ) M-1 at pH 8.3 .
	manualset3
244240	1	422165	7	NULL	NULL	0	NULL	Work	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Work and task load in old age ) .
	manualset3
244241	2	422165	7	NULL	NULL	0	NULL	task load	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Work and task load in old age ) .
	manualset3
244242	3	422165	7	NULL	NULL	0	NULL	old age	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	( Work and task load in old age ) .
	manualset3
244243	1	422166	7	NULL	NULL	0	NULL	Two main effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two main effects of wIRA on single cells are discussed : thermal effects , caused by absorption of energy by cellular water and the aqueous medium surrounding the irradiated sample that result in warming , and supposed athermal effects that result from a direct interaction of wIRA with cellular molecules/structures excluding water .
	manualset3
244244	2	422166	7	NULL	NULL	0	NULL	wIRA	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Two main effects of wIRA on single cells are discussed : thermal effects , caused by absorption of energy by cellular water and the aqueous medium surrounding the irradiated sample that result in warming , and supposed athermal effects that result from a direct interaction of wIRA with cellular molecules/structures excluding water .
	manualset3
244245	3	422166	7	NULL	NULL	0	NULL	 single cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Two main effects of wIRA on single cells are discussed : thermal effects , caused by absorption of energy by cellular water and the aqueous medium surrounding the irradiated sample that result in warming , and supposed athermal effects that result from a direct interaction of wIRA with cellular molecules/structures excluding water .
	manualset3
244246	4	422166	7	NULL	NULL	0	NULL	thermal effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two main effects of wIRA on single cells are discussed : thermal effects , caused by absorption of energy by cellular water and the aqueous medium surrounding the irradiated sample that result in warming , and supposed athermal effects that result from a direct interaction of wIRA with cellular molecules/structures excluding water .
	manualset3
244247	5	422166	7	NULL	NULL	0	NULL	absorption	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two main effects of wIRA on single cells are discussed : thermal effects , caused by absorption of energy by cellular water and the aqueous medium surrounding the irradiated sample that result in warming , and supposed athermal effects that result from a direct interaction of wIRA with cellular molecules/structures excluding water .
	manualset3
244248	6	422166	7	NULL	NULL	0	NULL	energy	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two main effects of wIRA on single cells are discussed : thermal effects , caused by absorption of energy by cellular water and the aqueous medium surrounding the irradiated sample that result in warming , and supposed athermal effects that result from a direct interaction of wIRA with cellular molecules/structures excluding water .
	manualset3
244249	7	422166	7	NULL	NULL	0	NULL	cellular water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two main effects of wIRA on single cells are discussed : thermal effects , caused by absorption of energy by cellular water and the aqueous medium surrounding the irradiated sample that result in warming , and supposed athermal effects that result from a direct interaction of wIRA with cellular molecules/structures excluding water .
	manualset3
244250	8	422166	7	NULL	NULL	0	NULL	aqueous medium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two main effects of wIRA on single cells are discussed : thermal effects , caused by absorption of energy by cellular water and the aqueous medium surrounding the irradiated sample that result in warming , and supposed athermal effects that result from a direct interaction of wIRA with cellular molecules/structures excluding water .
	manualset3
244251	9	422166	7	NULL	NULL	0	NULL	irradiated sample	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Two main effects of wIRA on single cells are discussed : thermal effects , caused by absorption of energy by cellular water and the aqueous medium surrounding the irradiated sample that result in warming , and supposed athermal effects that result from a direct interaction of wIRA with cellular molecules/structures excluding water .
	manualset3
244252	10	422166	7	NULL	NULL	0	NULL	warming	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two main effects of wIRA on single cells are discussed : thermal effects , caused by absorption of energy by cellular water and the aqueous medium surrounding the irradiated sample that result in warming , and supposed athermal effects that result from a direct interaction of wIRA with cellular molecules/structures excluding water .
	manualset3
244253	11	422166	7	NULL	NULL	0	NULL	athermal effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two main effects of wIRA on single cells are discussed : thermal effects , caused by absorption of energy by cellular water and the aqueous medium surrounding the irradiated sample that result in warming , and supposed athermal effects that result from a direct interaction of wIRA with cellular molecules/structures excluding water .
	manualset3
244254	12	422166	7	NULL	NULL	0	NULL	direct interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Two main effects of wIRA on single cells are discussed : thermal effects , caused by absorption of energy by cellular water and the aqueous medium surrounding the irradiated sample that result in warming , and supposed athermal effects that result from a direct interaction of wIRA with cellular molecules/structures excluding water .
	manualset3
244255	13	422166	7	NULL	NULL	0	NULL	 wIRA 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Two main effects of wIRA on single cells are discussed : thermal effects , caused by absorption of energy by cellular water and the aqueous medium surrounding the irradiated sample that result in warming , and supposed athermal effects that result from a direct interaction of wIRA with cellular molecules/structures excluding water .
	manualset3
244256	14	422166	7	NULL	NULL	0	NULL	cellular molecules/structures 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two main effects of wIRA on single cells are discussed : thermal effects , caused by absorption of energy by cellular water and the aqueous medium surrounding the irradiated sample that result in warming , and supposed athermal effects that result from a direct interaction of wIRA with cellular molecules/structures excluding water .
	manualset3
244257	15	422166	7	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Two main effects of wIRA on single cells are discussed : thermal effects , caused by absorption of energy by cellular water and the aqueous medium surrounding the irradiated sample that result in warming , and supposed athermal effects that result from a direct interaction of wIRA with cellular molecules/structures excluding water .
	manualset3
244258	1	422167	7	NULL	NULL	0	NULL	exfoliated oral cytology test 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An exfoliated oral cytology test for HPV was a significant predictor of HR types in the cancers , suggesting that an oral rinse may provide an early biomarker of infected tumors .
	manualset3
244259	2	422167	7	NULL	NULL	0	NULL	HPV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	An exfoliated oral cytology test for HPV was a significant predictor of HR types in the cancers , suggesting that an oral rinse may provide an early biomarker of infected tumors .
	manualset3
244260	3	422167	7	NULL	NULL	0	NULL	 predictor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An exfoliated oral cytology test for HPV was a significant predictor of HR types in the cancers , suggesting that an oral rinse may provide an early biomarker of infected tumors .
	manualset3
244261	4	422167	7	NULL	NULL	0	NULL	HR types	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	An exfoliated oral cytology test for HPV was a significant predictor of HR types in the cancers , suggesting that an oral rinse may provide an early biomarker of infected tumors .
	manualset3
244262	5	422167	7	NULL	NULL	0	NULL	cancers	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	An exfoliated oral cytology test for HPV was a significant predictor of HR types in the cancers , suggesting that an oral rinse may provide an early biomarker of infected tumors .
	manualset3
244263	6	422167	7	NULL	NULL	0	NULL	oral rinse	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An exfoliated oral cytology test for HPV was a significant predictor of HR types in the cancers , suggesting that an oral rinse may provide an early biomarker of infected tumors .
	manualset3
244264	7	422167	7	NULL	NULL	0	NULL	early biomarker 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An exfoliated oral cytology test for HPV was a significant predictor of HR types in the cancers , suggesting that an oral rinse may provide an early biomarker of infected tumors .
	manualset3
244265	8	422167	7	NULL	NULL	0	NULL	 infected tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An exfoliated oral cytology test for HPV was a significant predictor of HR types in the cancers , suggesting that an oral rinse may provide an early biomarker of infected tumors .
	manualset3
244266	1	422168	7	NULL	NULL	0	NULL	Cellular granules	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Cellular granules lacking boundary membranes harbor RNAs and their associated proteins and play diverse roles controlling the timing and location of protein synthesis .
	manualset3
244267	2	422168	7	NULL	NULL	0	NULL	membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Cellular granules lacking boundary membranes harbor RNAs and their associated proteins and play diverse roles controlling the timing and location of protein synthesis .
	manualset3
244268	3	422168	7	NULL	NULL	0	NULL	RNAs 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Cellular granules lacking boundary membranes harbor RNAs and their associated proteins and play diverse roles controlling the timing and location of protein synthesis .
	manualset3
244269	4	422168	7	NULL	NULL	0	NULL	associated proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Cellular granules lacking boundary membranes harbor RNAs and their associated proteins and play diverse roles controlling the timing and location of protein synthesis .
	manualset3
244270	5	422168	7	NULL	NULL	0	NULL	diverse roles	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cellular granules lacking boundary membranes harbor RNAs and their associated proteins and play diverse roles controlling the timing and location of protein synthesis .
	manualset3
244271	6	422168	7	NULL	NULL	0	NULL	timing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Cellular granules lacking boundary membranes harbor RNAs and their associated proteins and play diverse roles controlling the timing and location of protein synthesis .
	manualset3
244272	7	422168	7	NULL	NULL	0	NULL	location	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Cellular granules lacking boundary membranes harbor RNAs and their associated proteins and play diverse roles controlling the timing and location of protein synthesis .
	manualset3
244273	8	422168	7	NULL	NULL	0	NULL	protein synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cellular granules lacking boundary membranes harbor RNAs and their associated proteins and play diverse roles controlling the timing and location of protein synthesis .
	manualset3
244274	1	422169	7	NULL	NULL	0	NULL	1st stage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	1st stage of clot formation ) .
	manualset3
244275	2	422169	7	NULL	NULL	0	NULL	clot formation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	1st stage of clot formation ) .
	manualset3
244276	1	422170	7	NULL	NULL	0	NULL	 fresh gas flow	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The fresh gas flow was provided by a Jackson Rees modification of an Ayre 's T-piece and was determined according to the following formula : 3 x ( 1000 + ( 100 x body weight ) ) LPM .
	manualset3
244277	2	422170	7	NULL	NULL	0	NULL	Jackson Rees modification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The fresh gas flow was provided by a Jackson Rees modification of an Ayre 's T-piece and was determined according to the following formula : 3 x ( 1000 + ( 100 x body weight ) ) LPM .
	manualset3
244278	3	422170	7	NULL	NULL	0	NULL	Ayre 's T-piece	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The fresh gas flow was provided by a Jackson Rees modification of an Ayre 's T-piece and was determined according to the following formula : 3 x ( 1000 + ( 100 x body weight ) ) LPM .
	manualset3
244279	4	422170	7	NULL	NULL	0	NULL	formula	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The fresh gas flow was provided by a Jackson Rees modification of an Ayre 's T-piece and was determined according to the following formula : 3 x ( 1000 + ( 100 x body weight ) ) LPM .
	manualset3
244280	5	422170	7	NULL	NULL	0	NULL	3 x ( 1000 + ( 100 x body weight ) ) LPM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The fresh gas flow was provided by a Jackson Rees modification of an Ayre 's T-piece and was determined according to the following formula : 3 x ( 1000 + ( 100 x body weight ) ) LPM .
	manualset3
244281	1	422171	7	NULL	NULL	0	NULL	Effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Effect of left atrial compliance on pulmonary artery pressure : a case report .
	manualset3
244282	2	422171	7	NULL	NULL	0	NULL	left atrial compliance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Effect of left atrial compliance on pulmonary artery pressure : a case report .
	manualset3
244283	3	422171	7	NULL	NULL	0	NULL	pulmonary artery pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Effect of left atrial compliance on pulmonary artery pressure : a case report .
	manualset3
244284	4	422171	7	NULL	NULL	NULL	NULL	case report 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of left atrial compliance on pulmonary artery pressure : a case report .
	manualset3
244285	1	422172	7	NULL	NULL	0	NULL	Stimulus	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulus that induces sE-cad generation by ADAMs , MMPs , KLK7 , and plasmin in vitro ranges from serum withdrawal to pro-inflammatory cytokines to growth factors .
	manualset3
244286	2	422172	7	NULL	NULL	0	NULL	sE-cad generation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulus that induces sE-cad generation by ADAMs , MMPs , KLK7 , and plasmin in vitro ranges from serum withdrawal to pro-inflammatory cytokines to growth factors .
	manualset3
244287	3	422172	7	NULL	NULL	0	NULL	ADAMs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulus that induces sE-cad generation by ADAMs , MMPs , KLK7 , and plasmin in vitro ranges from serum withdrawal to pro-inflammatory cytokines to growth factors .
	manualset3
244288	4	422172	7	NULL	NULL	0	NULL	MMPs 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulus that induces sE-cad generation by ADAMs , MMPs , KLK7 , and plasmin in vitro ranges from serum withdrawal to pro-inflammatory cytokines to growth factors .
	manualset3
244289	5	422172	7	NULL	NULL	0	NULL	KLK7	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulus that induces sE-cad generation by ADAMs , MMPs , KLK7 , and plasmin in vitro ranges from serum withdrawal to pro-inflammatory cytokines to growth factors .
	manualset3
244290	6	422172	7	NULL	NULL	0	NULL	plasmin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulus that induces sE-cad generation by ADAMs , MMPs , KLK7 , and plasmin in vitro ranges from serum withdrawal to pro-inflammatory cytokines to growth factors .
	manualset3
244291	7	422172	7	NULL	NULL	0	NULL	serum withdrawal 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulus that induces sE-cad generation by ADAMs , MMPs , KLK7 , and plasmin in vitro ranges from serum withdrawal to pro-inflammatory cytokines to growth factors .
	manualset3
244292	8	422172	7	NULL	NULL	0	NULL	pro-inflammatory cytokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulus that induces sE-cad generation by ADAMs , MMPs , KLK7 , and plasmin in vitro ranges from serum withdrawal to pro-inflammatory cytokines to growth factors .
	manualset3
244293	9	422172	7	NULL	NULL	0	NULL	growth factors 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Stimulus that induces sE-cad generation by ADAMs , MMPs , KLK7 , and plasmin in vitro ranges from serum withdrawal to pro-inflammatory cytokines to growth factors .
	manualset3
244295	1	422173	7	NULL	NULL	0	NULL	Isolation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of the genomic sequence revealed that the gene covered a segment of 6 kb and spanned 11 exons from the translation initiation site ATG to the termination signal TGA .
	manualset3
244296	2	422173	7	NULL	NULL	0	NULL	genomic sequence 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of the genomic sequence revealed that the gene covered a segment of 6 kb and spanned 11 exons from the translation initiation site ATG to the termination signal TGA .
	manualset3
244297	3	422173	7	NULL	NULL	0	NULL	gene	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of the genomic sequence revealed that the gene covered a segment of 6 kb and spanned 11 exons from the translation initiation site ATG to the termination signal TGA .
	manualset3
244298	4	422173	7	NULL	NULL	0	NULL	segment	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of the genomic sequence revealed that the gene covered a segment of 6 kb and spanned 11 exons from the translation initiation site ATG to the termination signal TGA .
	manualset3
244299	5	422173	7	NULL	NULL	0	NULL	6 kb	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of the genomic sequence revealed that the gene covered a segment of 6 kb and spanned 11 exons from the translation initiation site ATG to the termination signal TGA .
	manualset3
244300	6	422173	7	NULL	NULL	NULL	NULL	spanned 11 exons	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Isolation of the genomic sequence revealed that the gene covered a segment of 6 kb and spanned 11 exons from the translation initiation site ATG to the termination signal TGA .
	manualset3
244301	7	422173	7	NULL	NULL	NULL	NULL	translation initiation site	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Isolation of the genomic sequence revealed that the gene covered a segment of 6 kb and spanned 11 exons from the translation initiation site ATG to the termination signal TGA .
	manualset3
244302	8	422173	7	NULL	NULL	0	NULL	ATG	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of the genomic sequence revealed that the gene covered a segment of 6 kb and spanned 11 exons from the translation initiation site ATG to the termination signal TGA .
	manualset3
244303	9	422173	7	NULL	NULL	NULL	NULL	termination signal	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Isolation of the genomic sequence revealed that the gene covered a segment of 6 kb and spanned 11 exons from the translation initiation site ATG to the termination signal TGA .
	manualset3
244304	10	422173	7	NULL	NULL	0	NULL	TGA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation of the genomic sequence revealed that the gene covered a segment of 6 kb and spanned 11 exons from the translation initiation site ATG to the termination signal TGA .
	manualset3
244305	1	422174	7	NULL	NULL	0	NULL	peripheries of lower limbs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The peripheries of lower limbs were measured at four regions ( A : end of tarsal bones , H : heel , B : immediately above the ankle , C : largest circumference of the calf ) at admission in 295 patients how CABG candidates and differences in these measurement points at discharge compared to measurements at admission time were calculated .
	manualset3
244306	2	422174	7	NULL	NULL	0	NULL	four regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The peripheries of lower limbs were measured at four regions ( A : end of tarsal bones , H : heel , B : immediately above the ankle , C : largest circumference of the calf ) at admission in 295 patients how CABG candidates and differences in these measurement points at discharge compared to measurements at admission time were calculated .
	manualset3
244308	4	422174	7	NULL	NULL	0	NULL	end of tarsal bones	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The peripheries of lower limbs were measured at four regions ( A : end of tarsal bones , H : heel , B : immediately above the ankle , C : largest circumference of the calf ) at admission in 295 patients how CABG candidates and differences in these measurement points at discharge compared to measurements at admission time were calculated .
	manualset3
244309	5	422174	7	NULL	NULL	NULL	NULL	 heel	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The peripheries of lower limbs were measured at four regions ( A : end of tarsal bones , H : heel , B : immediately above the ankle , C : largest circumference of the calf ) at admission in 295 patients how CABG candidates and differences in these measurement points at discharge compared to measurements at admission time were calculated .
	manualset3
244310	6	422174	7	NULL	NULL	0	NULL	immediately above the ankle	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The peripheries of lower limbs were measured at four regions ( A : end of tarsal bones , H : heel , B : immediately above the ankle , C : largest circumference of the calf ) at admission in 295 patients how CABG candidates and differences in these measurement points at discharge compared to measurements at admission time were calculated .
	manualset3
244311	7	422174	7	NULL	NULL	0	NULL	largest circumference of the calf	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The peripheries of lower limbs were measured at four regions ( A : end of tarsal bones , H : heel , B : immediately above the ankle , C : largest circumference of the calf ) at admission in 295 patients how CABG candidates and differences in these measurement points at discharge compared to measurements at admission time were calculated .
	manualset3
244312	8	422174	7	NULL	NULL	0	NULL	admission	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The peripheries of lower limbs were measured at four regions ( A : end of tarsal bones , H : heel , B : immediately above the ankle , C : largest circumference of the calf ) at admission in 295 patients how CABG candidates and differences in these measurement points at discharge compared to measurements at admission time were calculated .
	manualset3
244313	9	422174	7	NULL	NULL	0	NULL	295 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The peripheries of lower limbs were measured at four regions ( A : end of tarsal bones , H : heel , B : immediately above the ankle , C : largest circumference of the calf ) at admission in 295 patients how CABG candidates and differences in these measurement points at discharge compared to measurements at admission time were calculated .
	manualset3
244314	10	422174	7	NULL	NULL	0	NULL	CABG candidates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The peripheries of lower limbs were measured at four regions ( A : end of tarsal bones , H : heel , B : immediately above the ankle , C : largest circumference of the calf ) at admission in 295 patients how CABG candidates and differences in these measurement points at discharge compared to measurements at admission time were calculated .
	manualset3
244315	11	422174	7	NULL	NULL	0	NULL	measurement points 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The peripheries of lower limbs were measured at four regions ( A : end of tarsal bones , H : heel , B : immediately above the ankle , C : largest circumference of the calf ) at admission in 295 patients how CABG candidates and differences in these measurement points at discharge compared to measurements at admission time were calculated .
	manualset3
244316	12	422174	7	NULL	NULL	0	NULL	discharge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The peripheries of lower limbs were measured at four regions ( A : end of tarsal bones , H : heel , B : immediately above the ankle , C : largest circumference of the calf ) at admission in 295 patients how CABG candidates and differences in these measurement points at discharge compared to measurements at admission time were calculated .
	manualset3
244317	13	422174	7	NULL	NULL	0	NULL	measurements	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The peripheries of lower limbs were measured at four regions ( A : end of tarsal bones , H : heel , B : immediately above the ankle , C : largest circumference of the calf ) at admission in 295 patients how CABG candidates and differences in these measurement points at discharge compared to measurements at admission time were calculated .
	manualset3
244318	14	422174	7	NULL	NULL	0	NULL	admission time	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	The peripheries of lower limbs were measured at four regions ( A : end of tarsal bones , H : heel , B : immediately above the ankle , C : largest circumference of the calf ) at admission in 295 patients how CABG candidates and differences in these measurement points at discharge compared to measurements at admission time were calculated .
	manualset3
244319	1	422175	7	NULL	NULL	0	NULL	2-mercaptoethanol test	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( The 2-mercaptoethanol test in the early diagnosis of rubella ) .
	manualset3
244320	2	422175	7	NULL	NULL	0	NULL	early diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( The 2-mercaptoethanol test in the early diagnosis of rubella ) .
	manualset3
244321	3	422175	7	NULL	NULL	0	NULL	rubella	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( The 2-mercaptoethanol test in the early diagnosis of rubella ) .
	manualset3
244337	1	422176	7	NULL	NULL	0	NULL	measurements	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An experiment was conducted , making similar measurements , on 84 cows to compare two configurations for U.S. cubicles ( cantilevered on a double head rail as observed in the survey with a high and rear neck rail vs. fixed on freestanding posts as recommended ) and another recent cubicle type ( Euroconfort , cantilevered on head rails , but with a large space between the rails and fixed as recommended ) , with and without a brisket board .
	manualset3
244338	2	422176	7	NULL	NULL	0	NULL	 84 cows	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	An experiment was conducted , making similar measurements , on 84 cows to compare two configurations for U.S. cubicles ( cantilevered on a double head rail as observed in the survey with a high and rear neck rail vs. fixed on freestanding posts as recommended ) and another recent cubicle type ( Euroconfort , cantilevered on head rails , but with a large space between the rails and fixed as recommended ) , with and without a brisket board .
	manualset3
244339	3	422176	7	NULL	NULL	0	NULL	two configurations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An experiment was conducted , making similar measurements , on 84 cows to compare two configurations for U.S. cubicles ( cantilevered on a double head rail as observed in the survey with a high and rear neck rail vs. fixed on freestanding posts as recommended ) and another recent cubicle type ( Euroconfort , cantilevered on head rails , but with a large space between the rails and fixed as recommended ) , with and without a brisket board .
	manualset3
244340	4	422176	7	NULL	NULL	0	NULL	U.S. cubicles	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	An experiment was conducted , making similar measurements , on 84 cows to compare two configurations for U.S. cubicles ( cantilevered on a double head rail as observed in the survey with a high and rear neck rail vs. fixed on freestanding posts as recommended ) and another recent cubicle type ( Euroconfort , cantilevered on head rails , but with a large space between the rails and fixed as recommended ) , with and without a brisket board .
	manualset3
244341	5	422176	7	NULL	NULL	0	NULL	double head rail 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	An experiment was conducted , making similar measurements , on 84 cows to compare two configurations for U.S. cubicles ( cantilevered on a double head rail as observed in the survey with a high and rear neck rail vs. fixed on freestanding posts as recommended ) and another recent cubicle type ( Euroconfort , cantilevered on head rails , but with a large space between the rails and fixed as recommended ) , with and without a brisket board .
	manualset3
244342	6	422176	7	NULL	NULL	0	NULL	survey 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	An experiment was conducted , making similar measurements , on 84 cows to compare two configurations for U.S. cubicles ( cantilevered on a double head rail as observed in the survey with a high and rear neck rail vs. fixed on freestanding posts as recommended ) and another recent cubicle type ( Euroconfort , cantilevered on head rails , but with a large space between the rails and fixed as recommended ) , with and without a brisket board .
	manualset3
244343	7	422176	7	NULL	NULL	0	NULL	rear neck rail	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	An experiment was conducted , making similar measurements , on 84 cows to compare two configurations for U.S. cubicles ( cantilevered on a double head rail as observed in the survey with a high and rear neck rail vs. fixed on freestanding posts as recommended ) and another recent cubicle type ( Euroconfort , cantilevered on head rails , but with a large space between the rails and fixed as recommended ) , with and without a brisket board .
	manualset3
244344	8	422176	7	NULL	NULL	0	NULL	 freestanding posts	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	An experiment was conducted , making similar measurements , on 84 cows to compare two configurations for U.S. cubicles ( cantilevered on a double head rail as observed in the survey with a high and rear neck rail vs. fixed on freestanding posts as recommended ) and another recent cubicle type ( Euroconfort , cantilevered on head rails , but with a large space between the rails and fixed as recommended ) , with and without a brisket board .
	manualset3
244345	9	422176	7	NULL	NULL	0	NULL	cubicle type	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	An experiment was conducted , making similar measurements , on 84 cows to compare two configurations for U.S. cubicles ( cantilevered on a double head rail as observed in the survey with a high and rear neck rail vs. fixed on freestanding posts as recommended ) and another recent cubicle type ( Euroconfort , cantilevered on head rails , but with a large space between the rails and fixed as recommended ) , with and without a brisket board .
	manualset3
244346	10	422176	7	NULL	NULL	0	NULL	Euroconfort	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	An experiment was conducted , making similar measurements , on 84 cows to compare two configurations for U.S. cubicles ( cantilevered on a double head rail as observed in the survey with a high and rear neck rail vs. fixed on freestanding posts as recommended ) and another recent cubicle type ( Euroconfort , cantilevered on head rails , but with a large space between the rails and fixed as recommended ) , with and without a brisket board .
	manualset3
244347	11	422176	7	NULL	NULL	0	NULL	head rails	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	An experiment was conducted , making similar measurements , on 84 cows to compare two configurations for U.S. cubicles ( cantilevered on a double head rail as observed in the survey with a high and rear neck rail vs. fixed on freestanding posts as recommended ) and another recent cubicle type ( Euroconfort , cantilevered on head rails , but with a large space between the rails and fixed as recommended ) , with and without a brisket board .
	manualset3
244348	12	422176	7	NULL	NULL	0	NULL	large space 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	An experiment was conducted , making similar measurements , on 84 cows to compare two configurations for U.S. cubicles ( cantilevered on a double head rail as observed in the survey with a high and rear neck rail vs. fixed on freestanding posts as recommended ) and another recent cubicle type ( Euroconfort , cantilevered on head rails , but with a large space between the rails and fixed as recommended ) , with and without a brisket board .
	manualset3
244349	13	422176	7	NULL	NULL	0	NULL	rails	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	An experiment was conducted , making similar measurements , on 84 cows to compare two configurations for U.S. cubicles ( cantilevered on a double head rail as observed in the survey with a high and rear neck rail vs. fixed on freestanding posts as recommended ) and another recent cubicle type ( Euroconfort , cantilevered on head rails , but with a large space between the rails and fixed as recommended ) , with and without a brisket board .
	manualset3
244350	14	422176	7	NULL	NULL	0	NULL	brisket board	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	An experiment was conducted , making similar measurements , on 84 cows to compare two configurations for U.S. cubicles ( cantilevered on a double head rail as observed in the survey with a high and rear neck rail vs. fixed on freestanding posts as recommended ) and another recent cubicle type ( Euroconfort , cantilevered on head rails , but with a large space between the rails and fixed as recommended ) , with and without a brisket board .
	manualset3
245783	15	422176	7	NULL	NULL	0	NULL	experiment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An experiment was conducted , making similar measurements , on 84 cows to compare two configurations for U.S. cubicles ( cantilevered on a double head rail as observed in the survey with a high and rear neck rail vs. fixed on freestanding posts as recommended ) and another recent cubicle type ( Euroconfort , cantilevered on head rails , but with a large space between the rails and fixed as recommended ) , with and without a brisket board .
	manualset3
244351	1	422177	7	NULL	NULL	0	NULL	Bone grafts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Bone grafts from radius served as the graft and were positioned beneath the mandibular basis .
	manualset3
244352	2	422177	7	NULL	NULL	0	NULL	radius	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Bone grafts from radius served as the graft and were positioned beneath the mandibular basis .
	manualset3
244353	3	422177	7	NULL	NULL	0	NULL	graft 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Bone grafts from radius served as the graft and were positioned beneath the mandibular basis .
	manualset3
244354	4	422177	7	NULL	NULL	0	NULL	 mandibular basis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Bone grafts from radius served as the graft and were positioned beneath the mandibular basis .
	manualset3
244355	1	422178	7	NULL	NULL	0	NULL	Stark shift 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We have calculated the Stark shift of the exciton peak as a function of the local field for different silver thicknesses and various sizes of quantum dots based on the effective-mass Hamiltonian using the numerical-matrix-diagonalization method .
	manualset3
244356	2	422178	7	NULL	NULL	0	NULL	exciton peak	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We have calculated the Stark shift of the exciton peak as a function of the local field for different silver thicknesses and various sizes of quantum dots based on the effective-mass Hamiltonian using the numerical-matrix-diagonalization method .
	manualset3
244357	3	422178	7	NULL	NULL	0	NULL	 function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We have calculated the Stark shift of the exciton peak as a function of the local field for different silver thicknesses and various sizes of quantum dots based on the effective-mass Hamiltonian using the numerical-matrix-diagonalization method .
	manualset3
244358	4	422178	7	NULL	NULL	0	NULL	local field	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We have calculated the Stark shift of the exciton peak as a function of the local field for different silver thicknesses and various sizes of quantum dots based on the effective-mass Hamiltonian using the numerical-matrix-diagonalization method .
	manualset3
244359	5	422178	7	NULL	NULL	0	NULL	different silver thicknesses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We have calculated the Stark shift of the exciton peak as a function of the local field for different silver thicknesses and various sizes of quantum dots based on the effective-mass Hamiltonian using the numerical-matrix-diagonalization method .
	manualset3
244360	6	422178	7	NULL	NULL	0	NULL	various sizes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	We have calculated the Stark shift of the exciton peak as a function of the local field for different silver thicknesses and various sizes of quantum dots based on the effective-mass Hamiltonian using the numerical-matrix-diagonalization method .
	manualset3
244361	7	422178	7	NULL	NULL	0	NULL	quantum dots	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	We have calculated the Stark shift of the exciton peak as a function of the local field for different silver thicknesses and various sizes of quantum dots based on the effective-mass Hamiltonian using the numerical-matrix-diagonalization method .
	manualset3
244362	8	422178	7	NULL	NULL	0	NULL	effective-mass Hamiltonian 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We have calculated the Stark shift of the exciton peak as a function of the local field for different silver thicknesses and various sizes of quantum dots based on the effective-mass Hamiltonian using the numerical-matrix-diagonalization method .
	manualset3
244363	9	422178	7	NULL	NULL	0	NULL	numerical-matrix-diagonalization method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We have calculated the Stark shift of the exciton peak as a function of the local field for different silver thicknesses and various sizes of quantum dots based on the effective-mass Hamiltonian using the numerical-matrix-diagonalization method .
	manualset3
244364	1	422179	7	NULL	NULL	0	NULL	Orthostatic tolerance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Orthostatic tolerance was determined using a progressive lower-body negative pressure ( LBNP ) tolerance test before HDBR during normothermic conditions and on day 16 or day 18 of 6 HDBR during normothermic and skin surface cooling conditions ( randomized order post-HDBR ) .
	manualset3
244365	2	422179	7	NULL	NULL	0	NULL	progressive lower-body negative pressure ( LBNP ) tolerance test 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Orthostatic tolerance was determined using a progressive lower-body negative pressure ( LBNP ) tolerance test before HDBR during normothermic conditions and on day 16 or day 18 of 6 HDBR during normothermic and skin surface cooling conditions ( randomized order post-HDBR ) .
	manualset3
244366	3	422179	7	NULL	NULL	0	NULL	HDBR	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Orthostatic tolerance was determined using a progressive lower-body negative pressure ( LBNP ) tolerance test before HDBR during normothermic conditions and on day 16 or day 18 of 6 HDBR during normothermic and skin surface cooling conditions ( randomized order post-HDBR ) .
	manualset3
244367	4	422179	7	NULL	NULL	0	NULL	normothermic conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Orthostatic tolerance was determined using a progressive lower-body negative pressure ( LBNP ) tolerance test before HDBR during normothermic conditions and on day 16 or day 18 of 6 HDBR during normothermic and skin surface cooling conditions ( randomized order post-HDBR ) .
	manualset3
244368	5	422179	7	NULL	NULL	0	NULL	day 16 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Orthostatic tolerance was determined using a progressive lower-body negative pressure ( LBNP ) tolerance test before HDBR during normothermic conditions and on day 16 or day 18 of 6 HDBR during normothermic and skin surface cooling conditions ( randomized order post-HDBR ) .
	manualset3
244369	6	422179	7	NULL	NULL	0	NULL	day 18	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Orthostatic tolerance was determined using a progressive lower-body negative pressure ( LBNP ) tolerance test before HDBR during normothermic conditions and on day 16 or day 18 of 6 HDBR during normothermic and skin surface cooling conditions ( randomized order post-HDBR ) .
	manualset3
244370	7	422179	7	NULL	NULL	0	NULL	6 HDBR	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Orthostatic tolerance was determined using a progressive lower-body negative pressure ( LBNP ) tolerance test before HDBR during normothermic conditions and on day 16 or day 18 of 6 HDBR during normothermic and skin surface cooling conditions ( randomized order post-HDBR ) .
	manualset3
244371	8	422179	7	NULL	NULL	0	NULL	 normothermic conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Orthostatic tolerance was determined using a progressive lower-body negative pressure ( LBNP ) tolerance test before HDBR during normothermic conditions and on day 16 or day 18 of 6 HDBR during normothermic and skin surface cooling conditions ( randomized order post-HDBR ) .
	manualset3
244372	9	422179	7	NULL	NULL	0	NULL	 skin surface cooling conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Orthostatic tolerance was determined using a progressive lower-body negative pressure ( LBNP ) tolerance test before HDBR during normothermic conditions and on day 16 or day 18 of 6 HDBR during normothermic and skin surface cooling conditions ( randomized order post-HDBR ) .
	manualset3
244373	10	422179	7	NULL	NULL	0	NULL	post-HDBR	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Orthostatic tolerance was determined using a progressive lower-body negative pressure ( LBNP ) tolerance test before HDBR during normothermic conditions and on day 16 or day 18 of 6 HDBR during normothermic and skin surface cooling conditions ( randomized order post-HDBR ) .
	manualset3
244374	1	422180	7	NULL	NULL	0	NULL	microscopic 0.15 cm	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	A microscopic 0.15 cm thymoma ( microthymoma ) was incidentally found in the thymus during surgery .
	manualset3
244375	2	422180	7	NULL	NULL	0	NULL	thymoma ( microthymoma )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	A microscopic 0.15 cm thymoma ( microthymoma ) was incidentally found in the thymus during surgery .
	manualset3
244376	3	422180	7	NULL	NULL	0	NULL	thymus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	A microscopic 0.15 cm thymoma ( microthymoma ) was incidentally found in the thymus during surgery .
	manualset3
244377	4	422180	7	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	A microscopic 0.15 cm thymoma ( microthymoma ) was incidentally found in the thymus during surgery .
	manualset3
244378	1	422181	7	NULL	NULL	0	NULL	Investigation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of antigenic determinants of the microaerophilic obligate intracellular bacterium Lawsonia intracellularis using a mass spectrometry approach identified a novel bacterial protein present in an extract of cell culture medium aspirated from heavily infected in vitro cell cultures .
	manualset3
244379	2	422181	7	NULL	NULL	0	NULL	antigenic determinants	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of antigenic determinants of the microaerophilic obligate intracellular bacterium Lawsonia intracellularis using a mass spectrometry approach identified a novel bacterial protein present in an extract of cell culture medium aspirated from heavily infected in vitro cell cultures .
	manualset3
244380	3	422181	7	NULL	NULL	0	NULL	microaerophilic obligate intracellular bacterium	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of antigenic determinants of the microaerophilic obligate intracellular bacterium Lawsonia intracellularis using a mass spectrometry approach identified a novel bacterial protein present in an extract of cell culture medium aspirated from heavily infected in vitro cell cultures .
	manualset3
244381	4	422181	7	NULL	NULL	0	NULL	Lawsonia intracellularis 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of antigenic determinants of the microaerophilic obligate intracellular bacterium Lawsonia intracellularis using a mass spectrometry approach identified a novel bacterial protein present in an extract of cell culture medium aspirated from heavily infected in vitro cell cultures .
	manualset3
244382	5	422181	7	NULL	NULL	0	NULL	mass spectrometry approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of antigenic determinants of the microaerophilic obligate intracellular bacterium Lawsonia intracellularis using a mass spectrometry approach identified a novel bacterial protein present in an extract of cell culture medium aspirated from heavily infected in vitro cell cultures .
	manualset3
244383	6	422181	7	NULL	NULL	0	NULL	novel bacterial protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of antigenic determinants of the microaerophilic obligate intracellular bacterium Lawsonia intracellularis using a mass spectrometry approach identified a novel bacterial protein present in an extract of cell culture medium aspirated from heavily infected in vitro cell cultures .
	manualset3
244384	7	422181	7	NULL	NULL	NULL	NULL	extract	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Investigation of antigenic determinants of the microaerophilic obligate intracellular bacterium Lawsonia intracellularis using a mass spectrometry approach identified a novel bacterial protein present in an extract of cell culture medium aspirated from heavily infected in vitro cell cultures .
	manualset3
244385	8	422181	7	NULL	NULL	NULL	NULL	cell culture medium	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Investigation of antigenic determinants of the microaerophilic obligate intracellular bacterium Lawsonia intracellularis using a mass spectrometry approach identified a novel bacterial protein present in an extract of cell culture medium aspirated from heavily infected in vitro cell cultures .
	manualset3
244386	9	422181	7	NULL	NULL	0	NULL	heavily infected in vitro cell cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Investigation of antigenic determinants of the microaerophilic obligate intracellular bacterium Lawsonia intracellularis using a mass spectrometry approach identified a novel bacterial protein present in an extract of cell culture medium aspirated from heavily infected in vitro cell cultures .
	manualset3
244387	1	422182	7	NULL	NULL	0	NULL	E6123	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	E6123 inhibited PAF inhalation-induced bronchoconstriction in guinea pigs with an ED50 value ( p.o. ) of 1.3 micrograms/kg which was lower than those of other PAF-antagonists such as WEB2347 ( ED50 = 26 micrograms/kg ) and Y-24180 ( ED50 = 12 micrograms/kg ) .
	manualset3
244388	2	422182	7	NULL	NULL	0	NULL	PAF inhalation-induced bronchoconstriction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	E6123 inhibited PAF inhalation-induced bronchoconstriction in guinea pigs with an ED50 value ( p.o. ) of 1.3 micrograms/kg which was lower than those of other PAF-antagonists such as WEB2347 ( ED50 = 26 micrograms/kg ) and Y-24180 ( ED50 = 12 micrograms/kg ) .
	manualset3
244389	3	422182	7	NULL	NULL	0	NULL	guinea pigs 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	E6123 inhibited PAF inhalation-induced bronchoconstriction in guinea pigs with an ED50 value ( p.o. ) of 1.3 micrograms/kg which was lower than those of other PAF-antagonists such as WEB2347 ( ED50 = 26 micrograms/kg ) and Y-24180 ( ED50 = 12 micrograms/kg ) .
	manualset3
244390	4	422182	7	NULL	NULL	0	NULL	ED50 value ( p.o. )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	E6123 inhibited PAF inhalation-induced bronchoconstriction in guinea pigs with an ED50 value ( p.o. ) of 1.3 micrograms/kg which was lower than those of other PAF-antagonists such as WEB2347 ( ED50 = 26 micrograms/kg ) and Y-24180 ( ED50 = 12 micrograms/kg ) .
	manualset3
244391	5	422182	7	NULL	NULL	0	NULL	1.3 micrograms/kg	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	E6123 inhibited PAF inhalation-induced bronchoconstriction in guinea pigs with an ED50 value ( p.o. ) of 1.3 micrograms/kg which was lower than those of other PAF-antagonists such as WEB2347 ( ED50 = 26 micrograms/kg ) and Y-24180 ( ED50 = 12 micrograms/kg ) .
	manualset3
244392	6	422182	7	NULL	NULL	0	NULL	PAF-antagonists	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	E6123 inhibited PAF inhalation-induced bronchoconstriction in guinea pigs with an ED50 value ( p.o. ) of 1.3 micrograms/kg which was lower than those of other PAF-antagonists such as WEB2347 ( ED50 = 26 micrograms/kg ) and Y-24180 ( ED50 = 12 micrograms/kg ) .
	manualset3
244393	7	422182	7	NULL	NULL	0	NULL	WEB2347	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	E6123 inhibited PAF inhalation-induced bronchoconstriction in guinea pigs with an ED50 value ( p.o. ) of 1.3 micrograms/kg which was lower than those of other PAF-antagonists such as WEB2347 ( ED50 = 26 micrograms/kg ) and Y-24180 ( ED50 = 12 micrograms/kg ) .
	manualset3
244394	8	422182	7	NULL	NULL	0	NULL	ED50 = 26 micrograms/kg	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	E6123 inhibited PAF inhalation-induced bronchoconstriction in guinea pigs with an ED50 value ( p.o. ) of 1.3 micrograms/kg which was lower than those of other PAF-antagonists such as WEB2347 ( ED50 = 26 micrograms/kg ) and Y-24180 ( ED50 = 12 micrograms/kg ) .
	manualset3
244395	9	422182	7	NULL	NULL	0	NULL	Y-24180	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	E6123 inhibited PAF inhalation-induced bronchoconstriction in guinea pigs with an ED50 value ( p.o. ) of 1.3 micrograms/kg which was lower than those of other PAF-antagonists such as WEB2347 ( ED50 = 26 micrograms/kg ) and Y-24180 ( ED50 = 12 micrograms/kg ) .
	manualset3
244396	10	422182	7	NULL	NULL	0	NULL	ED50 = 12 micrograms/kg 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	E6123 inhibited PAF inhalation-induced bronchoconstriction in guinea pigs with an ED50 value ( p.o. ) of 1.3 micrograms/kg which was lower than those of other PAF-antagonists such as WEB2347 ( ED50 = 26 micrograms/kg ) and Y-24180 ( ED50 = 12 micrograms/kg ) .
	manualset3
244397	1	422183	7	NULL	NULL	0	NULL	 biogenesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The biogenesis of p51 , the target of nephritogenic monoclonal antibody 5-1-6 , was studied in the developing glomerulus by immunolocalization and metabolic labeling .
	manualset3
244398	2	422183	7	NULL	NULL	0	NULL	p51	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The biogenesis of p51 , the target of nephritogenic monoclonal antibody 5-1-6 , was studied in the developing glomerulus by immunolocalization and metabolic labeling .
	manualset3
244399	3	422183	7	NULL	NULL	0	NULL	target 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The biogenesis of p51 , the target of nephritogenic monoclonal antibody 5-1-6 , was studied in the developing glomerulus by immunolocalization and metabolic labeling .
	manualset3
244400	4	422183	7	NULL	NULL	0	NULL	nephritogenic monoclonal antibody 5-1-6	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The biogenesis of p51 , the target of nephritogenic monoclonal antibody 5-1-6 , was studied in the developing glomerulus by immunolocalization and metabolic labeling .
	manualset3
244401	5	422183	7	NULL	NULL	0	NULL	developing glomerulus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The biogenesis of p51 , the target of nephritogenic monoclonal antibody 5-1-6 , was studied in the developing glomerulus by immunolocalization and metabolic labeling .
	manualset3
244402	6	422183	7	NULL	NULL	0	NULL	immunolocalization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The biogenesis of p51 , the target of nephritogenic monoclonal antibody 5-1-6 , was studied in the developing glomerulus by immunolocalization and metabolic labeling .
	manualset3
244403	7	422183	7	NULL	NULL	0	NULL	metabolic labeling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The biogenesis of p51 , the target of nephritogenic monoclonal antibody 5-1-6 , was studied in the developing glomerulus by immunolocalization and metabolic labeling .
	manualset3
244404	1	422184	7	NULL	NULL	0	NULL	experimental approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An experimental approach to dreams and telepathy .
	manualset3
244405	2	422184	7	NULL	NULL	0	NULL	dreams	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An experimental approach to dreams and telepathy .
	manualset3
244406	3	422184	7	NULL	NULL	0	NULL	telepathy	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An experimental approach to dreams and telepathy .
	manualset3
244407	1	422185	7	NULL	NULL	0	NULL	immunofluorescence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunofluorescence in human lung sections was observed with the antibodies which were raised against GST psi and GST alpha-epsilon of human liver and GST pi of human placenta indicating that the isoenzymes corresponding to three gene loci , GST1 , GST2 , and GST3 are present in human lung .
	manualset3
244408	2	422185	7	NULL	NULL	0	NULL	human lung sections	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunofluorescence in human lung sections was observed with the antibodies which were raised against GST psi and GST alpha-epsilon of human liver and GST pi of human placenta indicating that the isoenzymes corresponding to three gene loci , GST1 , GST2 , and GST3 are present in human lung .
	manualset3
244409	3	422185	7	NULL	NULL	0	NULL	antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunofluorescence in human lung sections was observed with the antibodies which were raised against GST psi and GST alpha-epsilon of human liver and GST pi of human placenta indicating that the isoenzymes corresponding to three gene loci , GST1 , GST2 , and GST3 are present in human lung .
	manualset3
244410	4	422185	7	NULL	NULL	0	NULL	GST psi 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunofluorescence in human lung sections was observed with the antibodies which were raised against GST psi and GST alpha-epsilon of human liver and GST pi of human placenta indicating that the isoenzymes corresponding to three gene loci , GST1 , GST2 , and GST3 are present in human lung .
	manualset3
244411	5	422185	7	NULL	NULL	0	NULL	GST alpha-epsilon	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunofluorescence in human lung sections was observed with the antibodies which were raised against GST psi and GST alpha-epsilon of human liver and GST pi of human placenta indicating that the isoenzymes corresponding to three gene loci , GST1 , GST2 , and GST3 are present in human lung .
	manualset3
244412	6	422185	7	NULL	NULL	0	NULL	human liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunofluorescence in human lung sections was observed with the antibodies which were raised against GST psi and GST alpha-epsilon of human liver and GST pi of human placenta indicating that the isoenzymes corresponding to three gene loci , GST1 , GST2 , and GST3 are present in human lung .
	manualset3
244413	7	422185	7	NULL	NULL	0	NULL	GST pi 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunofluorescence in human lung sections was observed with the antibodies which were raised against GST psi and GST alpha-epsilon of human liver and GST pi of human placenta indicating that the isoenzymes corresponding to three gene loci , GST1 , GST2 , and GST3 are present in human lung .
	manualset3
244414	8	422185	7	NULL	NULL	0	NULL	human placenta 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunofluorescence in human lung sections was observed with the antibodies which were raised against GST psi and GST alpha-epsilon of human liver and GST pi of human placenta indicating that the isoenzymes corresponding to three gene loci , GST1 , GST2 , and GST3 are present in human lung .
	manualset3
244415	9	422185	7	NULL	NULL	0	NULL	isoenzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunofluorescence in human lung sections was observed with the antibodies which were raised against GST psi and GST alpha-epsilon of human liver and GST pi of human placenta indicating that the isoenzymes corresponding to three gene loci , GST1 , GST2 , and GST3 are present in human lung .
	manualset3
244416	10	422185	7	NULL	NULL	0	NULL	three gene loci 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunofluorescence in human lung sections was observed with the antibodies which were raised against GST psi and GST alpha-epsilon of human liver and GST pi of human placenta indicating that the isoenzymes corresponding to three gene loci , GST1 , GST2 , and GST3 are present in human lung .
	manualset3
244417	11	422185	7	NULL	NULL	0	NULL	GST1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunofluorescence in human lung sections was observed with the antibodies which were raised against GST psi and GST alpha-epsilon of human liver and GST pi of human placenta indicating that the isoenzymes corresponding to three gene loci , GST1 , GST2 , and GST3 are present in human lung .
	manualset3
244418	12	422185	7	NULL	NULL	0	NULL	 GST2	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunofluorescence in human lung sections was observed with the antibodies which were raised against GST psi and GST alpha-epsilon of human liver and GST pi of human placenta indicating that the isoenzymes corresponding to three gene loci , GST1 , GST2 , and GST3 are present in human lung .
	manualset3
244419	13	422185	7	NULL	NULL	0	NULL	GST3	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunofluorescence in human lung sections was observed with the antibodies which were raised against GST psi and GST alpha-epsilon of human liver and GST pi of human placenta indicating that the isoenzymes corresponding to three gene loci , GST1 , GST2 , and GST3 are present in human lung .
	manualset3
244420	14	422185	7	NULL	NULL	0	NULL	human lung	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The immunofluorescence in human lung sections was observed with the antibodies which were raised against GST psi and GST alpha-epsilon of human liver and GST pi of human placenta indicating that the isoenzymes corresponding to three gene loci , GST1 , GST2 , and GST3 are present in human lung .
	manualset3
244421	1	422186	7	NULL	NULL	0	NULL	Gastrointestinal foreign bodies	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Gastrointestinal foreign bodies of medical origin ) .
	manualset3
244422	2	422186	7	NULL	NULL	0	NULL	medical origin	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Gastrointestinal foreign bodies of medical origin ) .
	manualset3
244423	1	422187	7	NULL	NULL	0	NULL	 purified MnSOD	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The purified MnSOD of potato mitochondria was UV-cross-linked to the mitochondrial transcript .
	manualset3
244424	2	422187	7	NULL	NULL	0	NULL	 potato mitochondria	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The purified MnSOD of potato mitochondria was UV-cross-linked to the mitochondrial transcript .
	manualset3
244425	3	422187	7	NULL	NULL	0	NULL	mitochondrial transcript	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The purified MnSOD of potato mitochondria was UV-cross-linked to the mitochondrial transcript .
	manualset3
244426	1	422188	7	NULL	NULL	0	NULL	gamma scintigraphy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The gamma scintigraphy indicated that the microspheres cleared slowly from the nasal cavity .
	manualset3
244427	2	422188	7	NULL	NULL	0	NULL	microspheres	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The gamma scintigraphy indicated that the microspheres cleared slowly from the nasal cavity .
	manualset3
244428	3	422188	7	NULL	NULL	0	NULL	 nasal cavity	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The gamma scintigraphy indicated that the microspheres cleared slowly from the nasal cavity .
	manualset3
244429	1	422189	7	NULL	NULL	0	NULL	values 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The values obtained can be used to calculate the resulting polymer/solution interface activity of electrolyte ions , thus the detection limit of CP membrane can be theoretically predicted .
	manualset3
244430	2	422189	7	NULL	NULL	0	NULL	polymer/solution interface activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The values obtained can be used to calculate the resulting polymer/solution interface activity of electrolyte ions , thus the detection limit of CP membrane can be theoretically predicted .
	manualset3
244431	3	422189	7	NULL	NULL	0	NULL	electrolyte ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	The values obtained can be used to calculate the resulting polymer/solution interface activity of electrolyte ions , thus the detection limit of CP membrane can be theoretically predicted .
	manualset3
244432	4	422189	7	NULL	NULL	0	NULL	detection limit	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The values obtained can be used to calculate the resulting polymer/solution interface activity of electrolyte ions , thus the detection limit of CP membrane can be theoretically predicted .
	manualset3
244433	5	422189	7	NULL	NULL	0	NULL	CP membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The values obtained can be used to calculate the resulting polymer/solution interface activity of electrolyte ions , thus the detection limit of CP membrane can be theoretically predicted .
	manualset3
244434	1	422190	7	NULL	NULL	0	NULL	Endovascular treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Endovascular treatment of RAS is the technique of choice for most patients , whether diabetic or not .
	manualset3
244435	2	422190	7	NULL	NULL	0	NULL	RAS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Endovascular treatment of RAS is the technique of choice for most patients , whether diabetic or not .
	manualset3
244436	3	422190	7	NULL	NULL	0	NULL	technique	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Endovascular treatment of RAS is the technique of choice for most patients , whether diabetic or not .
	manualset3
244437	4	422190	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Endovascular treatment of RAS is the technique of choice for most patients , whether diabetic or not .
	manualset3
244438	1	422191	7	NULL	NULL	0	NULL	Report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Report of a WHO scientific group .
	manualset3
244439	2	422191	7	NULL	NULL	0	NULL	WHO scientific group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Report of a WHO scientific group .
	manualset3
244440	1	422192	7	NULL	NULL	0	NULL	Phospholipases A ( 2 ) ( PLA ( 2 ) ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospholipases A ( 2 ) ( PLA ( 2 ) ) hydrolyze the sn-2 fatty acid substituent , such as arachidonic acid , from phospholipids , and arachidonate metabolites are recognized mediators of bone modeling .
	manualset3
244441	2	422192	7	NULL	NULL	0	NULL	sn-2 fatty acid substituent	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospholipases A ( 2 ) ( PLA ( 2 ) ) hydrolyze the sn-2 fatty acid substituent , such as arachidonic acid , from phospholipids , and arachidonate metabolites are recognized mediators of bone modeling .
	manualset3
244442	3	422192	7	NULL	NULL	0	NULL	arachidonic acid	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospholipases A ( 2 ) ( PLA ( 2 ) ) hydrolyze the sn-2 fatty acid substituent , such as arachidonic acid , from phospholipids , and arachidonate metabolites are recognized mediators of bone modeling .
	manualset3
244443	4	422192	7	NULL	NULL	0	NULL	phospholipids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospholipases A ( 2 ) ( PLA ( 2 ) ) hydrolyze the sn-2 fatty acid substituent , such as arachidonic acid , from phospholipids , and arachidonate metabolites are recognized mediators of bone modeling .
	manualset3
244444	5	422192	7	NULL	NULL	0	NULL	arachidonate metabolites	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospholipases A ( 2 ) ( PLA ( 2 ) ) hydrolyze the sn-2 fatty acid substituent , such as arachidonic acid , from phospholipids , and arachidonate metabolites are recognized mediators of bone modeling .
	manualset3
244445	6	422192	7	NULL	NULL	0	NULL	mediators	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospholipases A ( 2 ) ( PLA ( 2 ) ) hydrolyze the sn-2 fatty acid substituent , such as arachidonic acid , from phospholipids , and arachidonate metabolites are recognized mediators of bone modeling .
	manualset3
244446	7	422192	7	NULL	NULL	0	NULL	bone modeling 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Phospholipases A ( 2 ) ( PLA ( 2 ) ) hydrolyze the sn-2 fatty acid substituent , such as arachidonic acid , from phospholipids , and arachidonate metabolites are recognized mediators of bone modeling .
	manualset3
244447	1	422193	7	NULL	NULL	0	NULL	Specialized AD/HD coaching	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specialized AD/HD coaching can be a helpful service for families and children .
	manualset3
244448	2	422193	7	NULL	NULL	0	NULL	service	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Specialized AD/HD coaching can be a helpful service for families and children .
	manualset3
244449	3	422193	7	NULL	NULL	0	NULL	families 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Specialized AD/HD coaching can be a helpful service for families and children .
	manualset3
244450	4	422193	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Specialized AD/HD coaching can be a helpful service for families and children .
	manualset3
244451	1	422194	7	NULL	NULL	0	NULL	Formamidopyrimidine-DNA glycosylase treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Formamidopyrimidine-DNA glycosylase treatment induced cleavage sites mainly at G residues of 5 ' - TG-3 ' sequence and at poly ( C ) sequences , in DNA incubated with BP-7 , 8 - dione in the presence of NADH and Cu ( II ) , whereas piperidine treatment induced cleavage sites at T mainly of 5 ' - TG-3 ' .
	manualset3
244452	2	422194	7	NULL	NULL	0	NULL	cleavage sites	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Formamidopyrimidine-DNA glycosylase treatment induced cleavage sites mainly at G residues of 5 ' - TG-3 ' sequence and at poly ( C ) sequences , in DNA incubated with BP-7 , 8 - dione in the presence of NADH and Cu ( II ) , whereas piperidine treatment induced cleavage sites at T mainly of 5 ' - TG-3 ' .
	manualset3
244453	3	422194	7	NULL	NULL	0	NULL	G residues	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Formamidopyrimidine-DNA glycosylase treatment induced cleavage sites mainly at G residues of 5 ' - TG-3 ' sequence and at poly ( C ) sequences , in DNA incubated with BP-7 , 8 - dione in the presence of NADH and Cu ( II ) , whereas piperidine treatment induced cleavage sites at T mainly of 5 ' - TG-3 ' .
	manualset3
244454	4	422194	7	NULL	NULL	0	NULL	5 ' - TG-3 ' sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Formamidopyrimidine-DNA glycosylase treatment induced cleavage sites mainly at G residues of 5 ' - TG-3 ' sequence and at poly ( C ) sequences , in DNA incubated with BP-7 , 8 - dione in the presence of NADH and Cu ( II ) , whereas piperidine treatment induced cleavage sites at T mainly of 5 ' - TG-3 ' .
	manualset3
244455	5	422194	7	NULL	NULL	0	NULL	 poly ( C ) sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Formamidopyrimidine-DNA glycosylase treatment induced cleavage sites mainly at G residues of 5 ' - TG-3 ' sequence and at poly ( C ) sequences , in DNA incubated with BP-7 , 8 - dione in the presence of NADH and Cu ( II ) , whereas piperidine treatment induced cleavage sites at T mainly of 5 ' - TG-3 ' .
	manualset3
244456	6	422194	7	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Formamidopyrimidine-DNA glycosylase treatment induced cleavage sites mainly at G residues of 5 ' - TG-3 ' sequence and at poly ( C ) sequences , in DNA incubated with BP-7 , 8 - dione in the presence of NADH and Cu ( II ) , whereas piperidine treatment induced cleavage sites at T mainly of 5 ' - TG-3 ' .
	manualset3
244457	7	422194	7	NULL	NULL	0	NULL	BP-7 , 8 - dione	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Formamidopyrimidine-DNA glycosylase treatment induced cleavage sites mainly at G residues of 5 ' - TG-3 ' sequence and at poly ( C ) sequences , in DNA incubated with BP-7 , 8 - dione in the presence of NADH and Cu ( II ) , whereas piperidine treatment induced cleavage sites at T mainly of 5 ' - TG-3 ' .
	manualset3
244458	8	422194	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Formamidopyrimidine-DNA glycosylase treatment induced cleavage sites mainly at G residues of 5 ' - TG-3 ' sequence and at poly ( C ) sequences , in DNA incubated with BP-7 , 8 - dione in the presence of NADH and Cu ( II ) , whereas piperidine treatment induced cleavage sites at T mainly of 5 ' - TG-3 ' .
	manualset3
244459	9	422194	7	NULL	NULL	0	NULL	NADH	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Formamidopyrimidine-DNA glycosylase treatment induced cleavage sites mainly at G residues of 5 ' - TG-3 ' sequence and at poly ( C ) sequences , in DNA incubated with BP-7 , 8 - dione in the presence of NADH and Cu ( II ) , whereas piperidine treatment induced cleavage sites at T mainly of 5 ' - TG-3 ' .
	manualset3
244460	10	422194	7	NULL	NULL	0	NULL	Cu ( II )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Formamidopyrimidine-DNA glycosylase treatment induced cleavage sites mainly at G residues of 5 ' - TG-3 ' sequence and at poly ( C ) sequences , in DNA incubated with BP-7 , 8 - dione in the presence of NADH and Cu ( II ) , whereas piperidine treatment induced cleavage sites at T mainly of 5 ' - TG-3 ' .
	manualset3
244461	11	422194	7	NULL	NULL	0	NULL	piperidine treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Formamidopyrimidine-DNA glycosylase treatment induced cleavage sites mainly at G residues of 5 ' - TG-3 ' sequence and at poly ( C ) sequences , in DNA incubated with BP-7 , 8 - dione in the presence of NADH and Cu ( II ) , whereas piperidine treatment induced cleavage sites at T mainly of 5 ' - TG-3 ' .
	manualset3
244462	12	422194	7	NULL	NULL	0	NULL	cleavage sites	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Formamidopyrimidine-DNA glycosylase treatment induced cleavage sites mainly at G residues of 5 ' - TG-3 ' sequence and at poly ( C ) sequences , in DNA incubated with BP-7 , 8 - dione in the presence of NADH and Cu ( II ) , whereas piperidine treatment induced cleavage sites at T mainly of 5 ' - TG-3 ' .
	manualset3
244463	13	422194	7	NULL	NULL	0	NULL	 T	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Formamidopyrimidine-DNA glycosylase treatment induced cleavage sites mainly at G residues of 5 ' - TG-3 ' sequence and at poly ( C ) sequences , in DNA incubated with BP-7 , 8 - dione in the presence of NADH and Cu ( II ) , whereas piperidine treatment induced cleavage sites at T mainly of 5 ' - TG-3 ' .
	manualset3
244464	14	422194	7	NULL	NULL	0	NULL	5 ' - TG-3 '	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Formamidopyrimidine-DNA glycosylase treatment induced cleavage sites mainly at G residues of 5 ' - TG-3 ' sequence and at poly ( C ) sequences , in DNA incubated with BP-7 , 8 - dione in the presence of NADH and Cu ( II ) , whereas piperidine treatment induced cleavage sites at T mainly of 5 ' - TG-3 ' .
	manualset3
244465	1	422195	7	NULL	NULL	NULL	NULL	Cytoid aggregates	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytoid aggregates of amyloid in the skin occur mainly in lichen amyloidosus and macular amyloidosis .
	manualset3
244466	2	422195	7	NULL	NULL	0	NULL	amyloid	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Cytoid aggregates of amyloid in the skin occur mainly in lichen amyloidosus and macular amyloidosis .
	manualset3
244467	3	422195	7	NULL	NULL	0	NULL	skin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Cytoid aggregates of amyloid in the skin occur mainly in lichen amyloidosus and macular amyloidosis .
	manualset3
244468	4	422195	7	NULL	NULL	0	NULL	lichen amyloidosus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Cytoid aggregates of amyloid in the skin occur mainly in lichen amyloidosus and macular amyloidosis .
	manualset3
244469	5	422195	7	NULL	NULL	0	NULL	macular amyloidosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Cytoid aggregates of amyloid in the skin occur mainly in lichen amyloidosus and macular amyloidosis .
	manualset3
244470	1	422196	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , antibody probes were used to screen a human placental expression library and cDNA clones isolated were characterized by polymerase chain reaction , Southern blot hybridisation , DNA cloning and partial nucleotide sequencing .
	manualset3
244471	2	422196	7	NULL	NULL	0	NULL	antibody probes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , antibody probes were used to screen a human placental expression library and cDNA clones isolated were characterized by polymerase chain reaction , Southern blot hybridisation , DNA cloning and partial nucleotide sequencing .
	manualset3
244472	3	422196	7	NULL	NULL	0	NULL	human placental expression library	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , antibody probes were used to screen a human placental expression library and cDNA clones isolated were characterized by polymerase chain reaction , Southern blot hybridisation , DNA cloning and partial nucleotide sequencing .
	manualset3
244473	4	422196	7	NULL	NULL	NULL	NULL	cDNA clones	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In this study , antibody probes were used to screen a human placental expression library and cDNA clones isolated were characterized by polymerase chain reaction , Southern blot hybridisation , DNA cloning and partial nucleotide sequencing .
	manualset3
244474	5	422196	7	NULL	NULL	0	NULL	polymerase chain reaction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , antibody probes were used to screen a human placental expression library and cDNA clones isolated were characterized by polymerase chain reaction , Southern blot hybridisation , DNA cloning and partial nucleotide sequencing .
	manualset3
244475	6	422196	7	NULL	NULL	0	NULL	Southern blot hybridisation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , antibody probes were used to screen a human placental expression library and cDNA clones isolated were characterized by polymerase chain reaction , Southern blot hybridisation , DNA cloning and partial nucleotide sequencing .
	manualset3
244476	7	422196	7	NULL	NULL	0	NULL	DNA cloning	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , antibody probes were used to screen a human placental expression library and cDNA clones isolated were characterized by polymerase chain reaction , Southern blot hybridisation , DNA cloning and partial nucleotide sequencing .
	manualset3
244477	8	422196	7	NULL	NULL	0	NULL	partial nucleotide sequencing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , antibody probes were used to screen a human placental expression library and cDNA clones isolated were characterized by polymerase chain reaction , Southern blot hybridisation , DNA cloning and partial nucleotide sequencing .
	manualset3
244478	1	422197	7	NULL	NULL	0	NULL	Clinics	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinics for spinal cord injuries .
	manualset3
244479	2	422197	7	NULL	NULL	0	NULL	spinal cord injuries	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Clinics for spinal cord injuries .
	manualset3
244480	1	422198	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We have now demonstrated the expression of both RFRP and its receptor ( GPR147 ) in primary cultures of human granulosa-lutein cells .
	manualset3
244481	2	422198	7	NULL	NULL	0	NULL	RFRP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We have now demonstrated the expression of both RFRP and its receptor ( GPR147 ) in primary cultures of human granulosa-lutein cells .
	manualset3
244482	3	422198	7	NULL	NULL	0	NULL	 receptor ( GPR147 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We have now demonstrated the expression of both RFRP and its receptor ( GPR147 ) in primary cultures of human granulosa-lutein cells .
	manualset3
244483	4	422198	7	NULL	NULL	0	NULL	primary cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We have now demonstrated the expression of both RFRP and its receptor ( GPR147 ) in primary cultures of human granulosa-lutein cells .
	manualset3
244484	5	422198	7	NULL	NULL	0	NULL	human granulosa-lutein cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We have now demonstrated the expression of both RFRP and its receptor ( GPR147 ) in primary cultures of human granulosa-lutein cells .
	manualset3
244485	1	422199	7	NULL	NULL	0	NULL	author	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	The author investigated the relationship between salient family processes and adolescent moral thought among a sample of 271 adolescents and their parents .
	manualset3
244486	2	422199	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The author investigated the relationship between salient family processes and adolescent moral thought among a sample of 271 adolescents and their parents .
	manualset3
244487	3	422199	7	NULL	NULL	0	NULL	salient family processes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The author investigated the relationship between salient family processes and adolescent moral thought among a sample of 271 adolescents and their parents .
	manualset3
244488	4	422199	7	NULL	NULL	0	NULL	adolescent moral thought 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The author investigated the relationship between salient family processes and adolescent moral thought among a sample of 271 adolescents and their parents .
	manualset3
244489	5	422199	7	NULL	NULL	0	NULL	sample	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The author investigated the relationship between salient family processes and adolescent moral thought among a sample of 271 adolescents and their parents .
	manualset3
244490	6	422199	7	NULL	NULL	0	NULL	271 adolescents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The author investigated the relationship between salient family processes and adolescent moral thought among a sample of 271 adolescents and their parents .
	manualset3
244491	7	422199	7	NULL	NULL	0	NULL	parents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The author investigated the relationship between salient family processes and adolescent moral thought among a sample of 271 adolescents and their parents .
	manualset3
244492	1	422200	7	NULL	NULL	0	NULL	Diabetic dermopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Diabetic dermopathy presents as well-demarcated , hyperpigmented , atrophic depressions , macules or papules located on the anterior surface of the lower legs of diabetic patients .
	manualset3
244493	2	422200	7	NULL	NULL	0	NULL	 atrophic depressions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Diabetic dermopathy presents as well-demarcated , hyperpigmented , atrophic depressions , macules or papules located on the anterior surface of the lower legs of diabetic patients .
	manualset3
244494	3	422200	7	NULL	NULL	0	NULL	macules	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Diabetic dermopathy presents as well-demarcated , hyperpigmented , atrophic depressions , macules or papules located on the anterior surface of the lower legs of diabetic patients .
	manualset3
244495	4	422200	7	NULL	NULL	0	NULL	papules	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Diabetic dermopathy presents as well-demarcated , hyperpigmented , atrophic depressions , macules or papules located on the anterior surface of the lower legs of diabetic patients .
	manualset3
244496	5	422200	7	NULL	NULL	0	NULL	anterior surface	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Diabetic dermopathy presents as well-demarcated , hyperpigmented , atrophic depressions , macules or papules located on the anterior surface of the lower legs of diabetic patients .
	manualset3
244497	6	422200	7	NULL	NULL	0	NULL	 lower legs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Diabetic dermopathy presents as well-demarcated , hyperpigmented , atrophic depressions , macules or papules located on the anterior surface of the lower legs of diabetic patients .
	manualset3
244498	7	422200	7	NULL	NULL	0	NULL	diabetic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Diabetic dermopathy presents as well-demarcated , hyperpigmented , atrophic depressions , macules or papules located on the anterior surface of the lower legs of diabetic patients .
	manualset3
244499	1	422201	7	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of contracting an STD was 4.2 times greater in those reporting sex with strangers ; 3.4 times greater in those with four or more sexual partners ; and 2.5 times greater in those reporting homosexual relations as compared with students not practicing such behaviors .
	manualset3
244500	2	422201	7	NULL	NULL	0	NULL	 STD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of contracting an STD was 4.2 times greater in those reporting sex with strangers ; 3.4 times greater in those with four or more sexual partners ; and 2.5 times greater in those reporting homosexual relations as compared with students not practicing such behaviors .
	manualset3
244501	3	422201	7	NULL	NULL	0	NULL	4.2 times	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of contracting an STD was 4.2 times greater in those reporting sex with strangers ; 3.4 times greater in those with four or more sexual partners ; and 2.5 times greater in those reporting homosexual relations as compared with students not practicing such behaviors .
	manualset3
244502	4	422201	7	NULL	NULL	0	NULL	 sex	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of contracting an STD was 4.2 times greater in those reporting sex with strangers ; 3.4 times greater in those with four or more sexual partners ; and 2.5 times greater in those reporting homosexual relations as compared with students not practicing such behaviors .
	manualset3
244503	5	422201	7	NULL	NULL	0	NULL	strangers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of contracting an STD was 4.2 times greater in those reporting sex with strangers ; 3.4 times greater in those with four or more sexual partners ; and 2.5 times greater in those reporting homosexual relations as compared with students not practicing such behaviors .
	manualset3
244504	6	422201	7	NULL	NULL	0	NULL	3.4 times	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of contracting an STD was 4.2 times greater in those reporting sex with strangers ; 3.4 times greater in those with four or more sexual partners ; and 2.5 times greater in those reporting homosexual relations as compared with students not practicing such behaviors .
	manualset3
244505	7	422201	7	NULL	NULL	0	NULL	four	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of contracting an STD was 4.2 times greater in those reporting sex with strangers ; 3.4 times greater in those with four or more sexual partners ; and 2.5 times greater in those reporting homosexual relations as compared with students not practicing such behaviors .
	manualset3
244506	8	422201	7	NULL	NULL	0	NULL	sexual partners	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of contracting an STD was 4.2 times greater in those reporting sex with strangers ; 3.4 times greater in those with four or more sexual partners ; and 2.5 times greater in those reporting homosexual relations as compared with students not practicing such behaviors .
	manualset3
244507	9	422201	7	NULL	NULL	0	NULL	2.5 times	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of contracting an STD was 4.2 times greater in those reporting sex with strangers ; 3.4 times greater in those with four or more sexual partners ; and 2.5 times greater in those reporting homosexual relations as compared with students not practicing such behaviors .
	manualset3
244508	10	422201	7	NULL	NULL	0	NULL	homosexual relations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of contracting an STD was 4.2 times greater in those reporting sex with strangers ; 3.4 times greater in those with four or more sexual partners ; and 2.5 times greater in those reporting homosexual relations as compared with students not practicing such behaviors .
	manualset3
244509	11	422201	7	NULL	NULL	0	NULL	students	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of contracting an STD was 4.2 times greater in those reporting sex with strangers ; 3.4 times greater in those with four or more sexual partners ; and 2.5 times greater in those reporting homosexual relations as compared with students not practicing such behaviors .
	manualset3
244510	12	422201	7	NULL	NULL	0	NULL	behaviors	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The risk of contracting an STD was 4.2 times greater in those reporting sex with strangers ; 3.4 times greater in those with four or more sexual partners ; and 2.5 times greater in those reporting homosexual relations as compared with students not practicing such behaviors .
	manualset3
244511	1	422202	7	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We have tested the hypothesis that the morphological abnormalities of the gastric mucosa in inactive ulcer disease are proportional to an alteration of the gastric luminal milieu itself due to abnormal secretory and motor function .
	manualset3
244512	2	422202	7	NULL	NULL	0	NULL	morphological abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We have tested the hypothesis that the morphological abnormalities of the gastric mucosa in inactive ulcer disease are proportional to an alteration of the gastric luminal milieu itself due to abnormal secretory and motor function .
	manualset3
244513	3	422202	7	NULL	NULL	0	NULL	gastric mucosa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We have tested the hypothesis that the morphological abnormalities of the gastric mucosa in inactive ulcer disease are proportional to an alteration of the gastric luminal milieu itself due to abnormal secretory and motor function .
	manualset3
244514	4	422202	7	NULL	NULL	0	NULL	inactive ulcer disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We have tested the hypothesis that the morphological abnormalities of the gastric mucosa in inactive ulcer disease are proportional to an alteration of the gastric luminal milieu itself due to abnormal secretory and motor function .
	manualset3
244515	5	422202	7	NULL	NULL	0	NULL	 alteration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We have tested the hypothesis that the morphological abnormalities of the gastric mucosa in inactive ulcer disease are proportional to an alteration of the gastric luminal milieu itself due to abnormal secretory and motor function .
	manualset3
244516	6	422202	7	NULL	NULL	0	NULL	gastric luminal milieu	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We have tested the hypothesis that the morphological abnormalities of the gastric mucosa in inactive ulcer disease are proportional to an alteration of the gastric luminal milieu itself due to abnormal secretory and motor function .
	manualset3
244517	7	422202	7	NULL	NULL	NULL	NULL	abnormal secretory function	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We have tested the hypothesis that the morphological abnormalities of the gastric mucosa in inactive ulcer disease are proportional to an alteration of the gastric luminal milieu itself due to abnormal secretory and motor function .
	manualset3
244518	8	422202	7	NULL	NULL	NULL	NULL	motor function	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We have tested the hypothesis that the morphological abnormalities of the gastric mucosa in inactive ulcer disease are proportional to an alteration of the gastric luminal milieu itself due to abnormal secretory and motor function .
	manualset3
244519	1	422203	7	NULL	NULL	0	NULL	short report 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This is a short report of a study based on a questionnaire answered by 477 young persons aged between 16 and 25 years , primarily with motor disabilities .
	manualset3
244520	2	422203	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This is a short report of a study based on a questionnaire answered by 477 young persons aged between 16 and 25 years , primarily with motor disabilities .
	manualset3
244521	3	422203	7	NULL	NULL	0	NULL	questionnaire	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This is a short report of a study based on a questionnaire answered by 477 young persons aged between 16 and 25 years , primarily with motor disabilities .
	manualset3
244522	4	422203	7	NULL	NULL	0	NULL	477 young persons	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This is a short report of a study based on a questionnaire answered by 477 young persons aged between 16 and 25 years , primarily with motor disabilities .
	manualset3
244523	5	422203	7	NULL	NULL	0	NULL	16 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	This is a short report of a study based on a questionnaire answered by 477 young persons aged between 16 and 25 years , primarily with motor disabilities .
	manualset3
244524	6	422203	7	NULL	NULL	0	NULL	25 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	This is a short report of a study based on a questionnaire answered by 477 young persons aged between 16 and 25 years , primarily with motor disabilities .
	manualset3
244525	7	422203	7	NULL	NULL	0	NULL	motor disabilities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This is a short report of a study based on a questionnaire answered by 477 young persons aged between 16 and 25 years , primarily with motor disabilities .
	manualset3
244526	1	422204	7	NULL	NULL	0	NULL	devices	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	These devices are a first step in the development of large-scale integrated ultrafast optical logic in silicon , and are two orders of magnitude faster than previously reported silicon devices .
	manualset3
244527	2	422204	7	NULL	NULL	0	NULL	first step	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These devices are a first step in the development of large-scale integrated ultrafast optical logic in silicon , and are two orders of magnitude faster than previously reported silicon devices .
	manualset3
244528	3	422204	7	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These devices are a first step in the development of large-scale integrated ultrafast optical logic in silicon , and are two orders of magnitude faster than previously reported silicon devices .
	manualset3
244529	4	422204	7	NULL	NULL	0	NULL	large-scale integrated ultrafast optical logic	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	These devices are a first step in the development of large-scale integrated ultrafast optical logic in silicon , and are two orders of magnitude faster than previously reported silicon devices .
	manualset3
244530	5	422204	7	NULL	NULL	0	NULL	silicon	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These devices are a first step in the development of large-scale integrated ultrafast optical logic in silicon , and are two orders of magnitude faster than previously reported silicon devices .
	manualset3
244531	6	422204	7	NULL	NULL	0	NULL	two orders	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These devices are a first step in the development of large-scale integrated ultrafast optical logic in silicon , and are two orders of magnitude faster than previously reported silicon devices .
	manualset3
244532	7	422204	7	NULL	NULL	0	NULL	magnitude	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These devices are a first step in the development of large-scale integrated ultrafast optical logic in silicon , and are two orders of magnitude faster than previously reported silicon devices .
	manualset3
244533	8	422204	7	NULL	NULL	0	NULL	silicon devices	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	These devices are a first step in the development of large-scale integrated ultrafast optical logic in silicon , and are two orders of magnitude faster than previously reported silicon devices .
	manualset3
244534	1	422205	7	NULL	NULL	0	NULL	seasonal fluctuations	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The seasonal fluctuations of the larval populations of four species of trichostrongylid nematode on pasture herbage .
	manualset3
244535	2	422205	7	NULL	NULL	0	NULL	larval populations	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The seasonal fluctuations of the larval populations of four species of trichostrongylid nematode on pasture herbage .
	manualset3
244536	3	422205	7	NULL	NULL	0	NULL	four species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The seasonal fluctuations of the larval populations of four species of trichostrongylid nematode on pasture herbage .
	manualset3
244537	4	422205	7	NULL	NULL	0	NULL	trichostrongylid nematode	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The seasonal fluctuations of the larval populations of four species of trichostrongylid nematode on pasture herbage .
	manualset3
244538	5	422205	7	NULL	NULL	0	NULL	 pasture herbage 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The seasonal fluctuations of the larval populations of four species of trichostrongylid nematode on pasture herbage .
	manualset3
244539	1	422206	7	NULL	NULL	0	NULL	Extracellular recordings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Extracellular recordings from IIN1c reveal sensory responses to ultrasonic ( ) 20 kHz ) , but not low frequency ( & lt ; 10 kHz ) sounds .
	manualset3
244540	2	422206	7	NULL	NULL	0	NULL	IIN1c	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Extracellular recordings from IIN1c reveal sensory responses to ultrasonic ( ) 20 kHz ) , but not low frequency ( & lt ; 10 kHz ) sounds .
	manualset3
244541	3	422206	7	NULL	NULL	NULL	NULL	sensory responses 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Extracellular recordings from IIN1c reveal sensory responses to ultrasonic ( ) 20 kHz ) , but not low frequency ( & lt ; 10 kHz ) sounds .
	manualset3
244542	4	422206	7	NULL	NULL	0	NULL	ultrasonic ( ) 20 kHz )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Extracellular recordings from IIN1c reveal sensory responses to ultrasonic ( ) 20 kHz ) , but not low frequency ( & lt ; 10 kHz ) sounds .
	manualset3
244543	5	422206	7	NULL	NULL	0	NULL	low frequency sounds	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Extracellular recordings from IIN1c reveal sensory responses to ultrasonic ( ) 20 kHz ) , but not low frequency ( & lt ; 10 kHz ) sounds .
	manualset3
244544	6	422206	7	NULL	NULL	0	NULL	& lt ; 10 kHz	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Extracellular recordings from IIN1c reveal sensory responses to ultrasonic ( ) 20 kHz ) , but not low frequency ( & lt ; 10 kHz ) sounds .
	manualset3
244545	1	422207	7	NULL	NULL	0	NULL	normal bladder	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with a normal bladder , a hyperplastic lesion exhibits a thickened , low scattering urothelium whereas a neoplastic lesion shows a thickened urothelium with increased backscattering .
	manualset3
244546	2	422207	7	NULL	NULL	0	NULL	hyperplastic lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with a normal bladder , a hyperplastic lesion exhibits a thickened , low scattering urothelium whereas a neoplastic lesion shows a thickened urothelium with increased backscattering .
	manualset3
244547	3	422207	7	NULL	NULL	0	NULL	thickened , low scattering urothelium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with a normal bladder , a hyperplastic lesion exhibits a thickened , low scattering urothelium whereas a neoplastic lesion shows a thickened urothelium with increased backscattering .
	manualset3
244548	4	422207	7	NULL	NULL	0	NULL	neoplastic lesion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with a normal bladder , a hyperplastic lesion exhibits a thickened , low scattering urothelium whereas a neoplastic lesion shows a thickened urothelium with increased backscattering .
	manualset3
244549	5	422207	7	NULL	NULL	0	NULL	thickened urothelium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with a normal bladder , a hyperplastic lesion exhibits a thickened , low scattering urothelium whereas a neoplastic lesion shows a thickened urothelium with increased backscattering .
	manualset3
244550	6	422207	7	NULL	NULL	0	NULL	backscattering	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with a normal bladder , a hyperplastic lesion exhibits a thickened , low scattering urothelium whereas a neoplastic lesion shows a thickened urothelium with increased backscattering .
	manualset3
244551	1	422208	7	NULL	NULL	0	NULL	Prevention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of recurrent urolithiasis is possible using an appropriate diet with or without medications .
	manualset3
244552	2	422208	7	NULL	NULL	0	NULL	 recurrent urolithiasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of recurrent urolithiasis is possible using an appropriate diet with or without medications .
	manualset3
244553	3	422208	7	NULL	NULL	0	NULL	diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of recurrent urolithiasis is possible using an appropriate diet with or without medications .
	manualset3
244554	4	422208	7	NULL	NULL	0	NULL	medications	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Prevention of recurrent urolithiasis is possible using an appropriate diet with or without medications .
	manualset3
244555	1	422209	7	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An exposure to a novel environment induced hyperexploratory behavior and elevated the level of free DOPAC in CSF in lesioned rats .
	manualset3
244556	2	422209	7	NULL	NULL	0	NULL	novel environment	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	An exposure to a novel environment induced hyperexploratory behavior and elevated the level of free DOPAC in CSF in lesioned rats .
	manualset3
244557	3	422209	7	NULL	NULL	0	NULL	hyperexploratory behavior 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An exposure to a novel environment induced hyperexploratory behavior and elevated the level of free DOPAC in CSF in lesioned rats .
	manualset3
244558	4	422209	7	NULL	NULL	0	NULL	level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An exposure to a novel environment induced hyperexploratory behavior and elevated the level of free DOPAC in CSF in lesioned rats .
	manualset3
244559	5	422209	7	NULL	NULL	0	NULL	free DOPAC	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An exposure to a novel environment induced hyperexploratory behavior and elevated the level of free DOPAC in CSF in lesioned rats .
	manualset3
244560	6	422209	7	NULL	NULL	0	NULL	 CSF	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An exposure to a novel environment induced hyperexploratory behavior and elevated the level of free DOPAC in CSF in lesioned rats .
	manualset3
244561	7	422209	7	NULL	NULL	0	NULL	lesioned rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	An exposure to a novel environment induced hyperexploratory behavior and elevated the level of free DOPAC in CSF in lesioned rats .
	manualset3
244562	1	422210	7	NULL	NULL	NULL	NULL	Surgical excision	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Surgical excision confirmed the diagnosis and resulted in resolution of the monoarthritis .
	manualset3
244563	2	422210	7	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Surgical excision confirmed the diagnosis and resulted in resolution of the monoarthritis .
	manualset3
244564	3	422210	7	NULL	NULL	0	NULL	resolution	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Surgical excision confirmed the diagnosis and resulted in resolution of the monoarthritis .
	manualset3
244565	4	422210	7	NULL	NULL	NULL	NULL	monoarthritis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Surgical excision confirmed the diagnosis and resulted in resolution of the monoarthritis .
	manualset3
244566	1	422211	7	NULL	NULL	0	NULL	Activity budgets	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity budgets and activity rhythms in red ruffed lemurs ( Varecia rubra ) on the Masoala Peninsula , Madagascar : seasonality and reproductive energetics .
	manualset3
244567	2	422211	7	NULL	NULL	0	NULL	activity rhythms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity budgets and activity rhythms in red ruffed lemurs ( Varecia rubra ) on the Masoala Peninsula , Madagascar : seasonality and reproductive energetics .
	manualset3
244568	3	422211	7	NULL	NULL	0	NULL	red ruffed lemurs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity budgets and activity rhythms in red ruffed lemurs ( Varecia rubra ) on the Masoala Peninsula , Madagascar : seasonality and reproductive energetics .
	manualset3
244569	4	422211	7	NULL	NULL	0	NULL	Varecia rubra	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity budgets and activity rhythms in red ruffed lemurs ( Varecia rubra ) on the Masoala Peninsula , Madagascar : seasonality and reproductive energetics .
	manualset3
244570	5	422211	7	NULL	NULL	0	NULL	Masoala Peninsula	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity budgets and activity rhythms in red ruffed lemurs ( Varecia rubra ) on the Masoala Peninsula , Madagascar : seasonality and reproductive energetics .
	manualset3
244571	6	422211	7	NULL	NULL	0	NULL	Madagascar	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity budgets and activity rhythms in red ruffed lemurs ( Varecia rubra ) on the Masoala Peninsula , Madagascar : seasonality and reproductive energetics .
	manualset3
244572	7	422211	7	NULL	NULL	0	NULL	seasonality	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity budgets and activity rhythms in red ruffed lemurs ( Varecia rubra ) on the Masoala Peninsula , Madagascar : seasonality and reproductive energetics .
	manualset3
244573	8	422211	7	NULL	NULL	0	NULL	reproductive energetics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Activity budgets and activity rhythms in red ruffed lemurs ( Varecia rubra ) on the Masoala Peninsula , Madagascar : seasonality and reproductive energetics .
	manualset3
244574	1	422212	7	NULL	NULL	0	NULL	Detection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Detection of proliferating hepatocytes by immunohistochemical staining for proliferating cell nuclear antigen ( PCNA ) in patients with acute hepatic failure .
	manualset3
244575	2	422212	7	NULL	NULL	0	NULL	proliferating hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Detection of proliferating hepatocytes by immunohistochemical staining for proliferating cell nuclear antigen ( PCNA ) in patients with acute hepatic failure .
	manualset3
244576	3	422212	7	NULL	NULL	0	NULL	immunohistochemical staining	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Detection of proliferating hepatocytes by immunohistochemical staining for proliferating cell nuclear antigen ( PCNA ) in patients with acute hepatic failure .
	manualset3
244577	4	422212	7	NULL	NULL	0	NULL	proliferating cell nuclear antigen ( PCNA )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Detection of proliferating hepatocytes by immunohistochemical staining for proliferating cell nuclear antigen ( PCNA ) in patients with acute hepatic failure .
	manualset3
244578	5	422212	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Detection of proliferating hepatocytes by immunohistochemical staining for proliferating cell nuclear antigen ( PCNA ) in patients with acute hepatic failure .
	manualset3
244579	6	422212	7	NULL	NULL	0	NULL	acute hepatic failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Detection of proliferating hepatocytes by immunohistochemical staining for proliferating cell nuclear antigen ( PCNA ) in patients with acute hepatic failure .
	manualset3
244580	1	422213	7	NULL	NULL	0	NULL	current strategies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The current strategies for acute cough management need to be reassessed , with a focus on developing new , reliable products and formulations with proven efficacy and safety .
	manualset3
244581	2	422213	7	NULL	NULL	0	NULL	acute cough management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The current strategies for acute cough management need to be reassessed , with a focus on developing new , reliable products and formulations with proven efficacy and safety .
	manualset3
244582	3	422213	7	NULL	NULL	0	NULL	reliable products	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The current strategies for acute cough management need to be reassessed , with a focus on developing new , reliable products and formulations with proven efficacy and safety .
	manualset3
244583	4	422213	7	NULL	NULL	0	NULL	formulations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The current strategies for acute cough management need to be reassessed , with a focus on developing new , reliable products and formulations with proven efficacy and safety .
	manualset3
244584	5	422213	7	NULL	NULL	0	NULL	safety	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The current strategies for acute cough management need to be reassessed , with a focus on developing new , reliable products and formulations with proven efficacy and safety .
	manualset3
244585	1	422214	7	NULL	NULL	0	NULL	histologic lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The predominant histologic lesions were interstitial nephritis , chronic tubular necrosis , lymphoplasmacytic infiltration within the kidney , liver , and pancreas , and focal non-suppurative encephalitis .
	manualset3
244586	2	422214	7	NULL	NULL	0	NULL	 interstitial nephritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The predominant histologic lesions were interstitial nephritis , chronic tubular necrosis , lymphoplasmacytic infiltration within the kidney , liver , and pancreas , and focal non-suppurative encephalitis .
	manualset3
244587	3	422214	7	NULL	NULL	0	NULL	chronic tubular necrosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The predominant histologic lesions were interstitial nephritis , chronic tubular necrosis , lymphoplasmacytic infiltration within the kidney , liver , and pancreas , and focal non-suppurative encephalitis .
	manualset3
244588	4	422214	7	NULL	NULL	0	NULL	 lymphoplasmacytic infiltration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The predominant histologic lesions were interstitial nephritis , chronic tubular necrosis , lymphoplasmacytic infiltration within the kidney , liver , and pancreas , and focal non-suppurative encephalitis .
	manualset3
244589	5	422214	7	NULL	NULL	0	NULL	kidney	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The predominant histologic lesions were interstitial nephritis , chronic tubular necrosis , lymphoplasmacytic infiltration within the kidney , liver , and pancreas , and focal non-suppurative encephalitis .
	manualset3
244590	6	422214	7	NULL	NULL	0	NULL	 liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The predominant histologic lesions were interstitial nephritis , chronic tubular necrosis , lymphoplasmacytic infiltration within the kidney , liver , and pancreas , and focal non-suppurative encephalitis .
	manualset3
244591	7	422214	7	NULL	NULL	0	NULL	pancreas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The predominant histologic lesions were interstitial nephritis , chronic tubular necrosis , lymphoplasmacytic infiltration within the kidney , liver , and pancreas , and focal non-suppurative encephalitis .
	manualset3
244592	8	422214	7	NULL	NULL	0	NULL	focal non-suppurative encephalitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The predominant histologic lesions were interstitial nephritis , chronic tubular necrosis , lymphoplasmacytic infiltration within the kidney , liver , and pancreas , and focal non-suppurative encephalitis .
	manualset3
244593	1	422215	7	NULL	NULL	0	NULL	4-Hydroxyphenylpyruvic acid dioxygenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	4-Hydroxyphenylpyruvic acid dioxygenase is an important enzyme in tyrosine catabolism in most organisms .
	manualset3
244594	2	422215	7	NULL	NULL	0	NULL	enzyme	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	4-Hydroxyphenylpyruvic acid dioxygenase is an important enzyme in tyrosine catabolism in most organisms .
	manualset3
244595	3	422215	7	NULL	NULL	0	NULL	tyrosine catabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	4-Hydroxyphenylpyruvic acid dioxygenase is an important enzyme in tyrosine catabolism in most organisms .
	manualset3
244596	4	422215	7	NULL	NULL	0	NULL	organisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	4-Hydroxyphenylpyruvic acid dioxygenase is an important enzyme in tyrosine catabolism in most organisms .
	manualset3
244597	1	422216	7	NULL	NULL	0	NULL	extended network	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An extended network of O-H ... O hydrogen bonds links the ( ISA ) ( - ) anions and the crystal water molecules .
	manualset3
244598	2	422216	7	NULL	NULL	0	NULL	O-H ... O hydrogen bonds	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An extended network of O-H ... O hydrogen bonds links the ( ISA ) ( - ) anions and the crystal water molecules .
	manualset3
244599	3	422216	7	NULL	NULL	0	NULL	( ISA ) ( - ) anions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	An extended network of O-H ... O hydrogen bonds links the ( ISA ) ( - ) anions and the crystal water molecules .
	manualset3
244600	4	422216	7	NULL	NULL	0	NULL	crystal water molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	An extended network of O-H ... O hydrogen bonds links the ( ISA ) ( - ) anions and the crystal water molecules .
	manualset3
244601	1	422217	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This study may provide a basis for the use of interspecific hybrid embryos of these organisms to investigate the evolution and importance of certain DNA sequences in early developmental processes leading to cell differentiation .
	manualset3
244602	2	422217	7	NULL	NULL	0	NULL	basis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This study may provide a basis for the use of interspecific hybrid embryos of these organisms to investigate the evolution and importance of certain DNA sequences in early developmental processes leading to cell differentiation .
	manualset3
244603	3	422217	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This study may provide a basis for the use of interspecific hybrid embryos of these organisms to investigate the evolution and importance of certain DNA sequences in early developmental processes leading to cell differentiation .
	manualset3
244604	4	422217	7	NULL	NULL	0	NULL	interspecific hybrid embryos	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	This study may provide a basis for the use of interspecific hybrid embryos of these organisms to investigate the evolution and importance of certain DNA sequences in early developmental processes leading to cell differentiation .
	manualset3
244605	5	422217	7	NULL	NULL	0	NULL	organisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	This study may provide a basis for the use of interspecific hybrid embryos of these organisms to investigate the evolution and importance of certain DNA sequences in early developmental processes leading to cell differentiation .
	manualset3
244606	6	422217	7	NULL	NULL	0	NULL	evolution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This study may provide a basis for the use of interspecific hybrid embryos of these organisms to investigate the evolution and importance of certain DNA sequences in early developmental processes leading to cell differentiation .
	manualset3
244607	7	422217	7	NULL	NULL	0	NULL	DNA sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	This study may provide a basis for the use of interspecific hybrid embryos of these organisms to investigate the evolution and importance of certain DNA sequences in early developmental processes leading to cell differentiation .
	manualset3
244608	8	422217	7	NULL	NULL	0	NULL	early developmental processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This study may provide a basis for the use of interspecific hybrid embryos of these organisms to investigate the evolution and importance of certain DNA sequences in early developmental processes leading to cell differentiation .
	manualset3
244609	9	422217	7	NULL	NULL	0	NULL	cell differentiation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This study may provide a basis for the use of interspecific hybrid embryos of these organisms to investigate the evolution and importance of certain DNA sequences in early developmental processes leading to cell differentiation .
	manualset3
244610	1	422218	7	NULL	NULL	0	NULL	Epstein-Barr virus nuclear antigen leader protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The Epstein-Barr virus nuclear antigen leader protein associates with hsp72/hsc73 .
	manualset3
244611	2	422218	7	NULL	NULL	0	NULL	hsp72/hsc73	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The Epstein-Barr virus nuclear antigen leader protein associates with hsp72/hsc73 .
	manualset3
244612	1	422219	7	NULL	NULL	0	NULL	 example	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These are , for example , CBM20s from hypothetical GH57 amylopullulanase ( probably lacking the starch-binding site 2 ) and CBM48s from the GH13 pullulanase subfamily ( probably lacking the starch/glycogen-binding site 1 ) .
	manualset3
244613	2	422219	7	NULL	NULL	NULL	NULL	CBM20s	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These are , for example , CBM20s from hypothetical GH57 amylopullulanase ( probably lacking the starch-binding site 2 ) and CBM48s from the GH13 pullulanase subfamily ( probably lacking the starch/glycogen-binding site 1 ) .
	manualset3
244614	3	422219	7	NULL	NULL	0	NULL	hypothetical GH57 amylopullulanase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	These are , for example , CBM20s from hypothetical GH57 amylopullulanase ( probably lacking the starch-binding site 2 ) and CBM48s from the GH13 pullulanase subfamily ( probably lacking the starch/glycogen-binding site 1 ) .
	manualset3
244615	4	422219	7	NULL	NULL	0	NULL	starch-binding site 2	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These are , for example , CBM20s from hypothetical GH57 amylopullulanase ( probably lacking the starch-binding site 2 ) and CBM48s from the GH13 pullulanase subfamily ( probably lacking the starch/glycogen-binding site 1 ) .
	manualset3
244616	5	422219	7	NULL	NULL	0	NULL	CBM48s	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These are , for example , CBM20s from hypothetical GH57 amylopullulanase ( probably lacking the starch-binding site 2 ) and CBM48s from the GH13 pullulanase subfamily ( probably lacking the starch/glycogen-binding site 1 ) .
	manualset3
244617	6	422219	7	NULL	NULL	0	NULL	GH13 pullulanase subfamily	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	These are , for example , CBM20s from hypothetical GH57 amylopullulanase ( probably lacking the starch-binding site 2 ) and CBM48s from the GH13 pullulanase subfamily ( probably lacking the starch/glycogen-binding site 1 ) .
	manualset3
244618	7	422219	7	NULL	NULL	0	NULL	starch/glycogen-binding site 1	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	These are , for example , CBM20s from hypothetical GH57 amylopullulanase ( probably lacking the starch-binding site 2 ) and CBM48s from the GH13 pullulanase subfamily ( probably lacking the starch/glycogen-binding site 1 ) .
	manualset3
244619	1	422220	7	NULL	NULL	0	NULL	 amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of bone resorption was determined by the condition imposed to the interface , being slightly larger when the interface was loose .
	manualset3
244620	2	422220	7	NULL	NULL	0	NULL	bone resorption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of bone resorption was determined by the condition imposed to the interface , being slightly larger when the interface was loose .
	manualset3
244621	3	422220	7	NULL	NULL	0	NULL	condition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of bone resorption was determined by the condition imposed to the interface , being slightly larger when the interface was loose .
	manualset3
244622	4	422220	7	NULL	NULL	0	NULL	 interface	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of bone resorption was determined by the condition imposed to the interface , being slightly larger when the interface was loose .
	manualset3
244623	5	422220	7	NULL	NULL	0	NULL	interface	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The amount of bone resorption was determined by the condition imposed to the interface , being slightly larger when the interface was loose .
	manualset3
244624	1	422221	7	NULL	NULL	0	NULL	Analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of cranial 133-Xenon clearance in the newborn infant by the two-compartment model .
	manualset3
244625	2	422221	7	NULL	NULL	0	NULL	cranial 133-Xenon clearance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of cranial 133-Xenon clearance in the newborn infant by the two-compartment model .
	manualset3
244626	3	422221	7	NULL	NULL	0	NULL	newborn infant	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of cranial 133-Xenon clearance in the newborn infant by the two-compartment model .
	manualset3
244627	4	422221	7	NULL	NULL	0	NULL	 two-compartment model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of cranial 133-Xenon clearance in the newborn infant by the two-compartment model .
	manualset3
244628	1	422222	7	NULL	NULL	0	NULL	abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Most conspicuous are abnormalities of megakaryopoiesis with regard to their histotopography and maturation .
	manualset3
244629	2	422222	7	NULL	NULL	0	NULL	megakaryopoiesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Most conspicuous are abnormalities of megakaryopoiesis with regard to their histotopography and maturation .
	manualset3
244630	3	422222	7	NULL	NULL	0	NULL	histotopography	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Most conspicuous are abnormalities of megakaryopoiesis with regard to their histotopography and maturation .
	manualset3
244631	4	422222	7	NULL	NULL	0	NULL	maturation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Most conspicuous are abnormalities of megakaryopoiesis with regard to their histotopography and maturation .
	manualset3
244632	1	422223	7	NULL	NULL	0	NULL	values 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The values were found to be P = -72 + / -6 % and P = 18 + / -7 % for CoS2 and Co0 .9 Fe0 .1 S2 , respectively .
	manualset3
244633	2	422223	7	NULL	NULL	0	NULL	P = -72 + / -6 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The values were found to be P = -72 + / -6 % and P = 18 + / -7 % for CoS2 and Co0 .9 Fe0 .1 S2 , respectively .
	manualset3
244634	3	422223	7	NULL	NULL	0	NULL	P = 18 + / -7 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The values were found to be P = -72 + / -6 % and P = 18 + / -7 % for CoS2 and Co0 .9 Fe0 .1 S2 , respectively .
	manualset3
244635	4	422223	7	NULL	NULL	0	NULL	CoS2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The values were found to be P = -72 + / -6 % and P = 18 + / -7 % for CoS2 and Co0 .9 Fe0 .1 S2 , respectively .
	manualset3
244636	5	422223	7	NULL	NULL	0	NULL	 Co0 .9 Fe0 .1 S2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The values were found to be P = -72 + / -6 % and P = 18 + / -7 % for CoS2 and Co0 .9 Fe0 .1 S2 , respectively .
	manualset3
244637	1	422224	7	NULL	NULL	0	NULL	Periodic lateralized epileptiform discharges	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Periodic lateralized epileptiform discharges -- long-term outcome in adults .
	manualset3
244638	2	422224	7	NULL	NULL	0	NULL	long-term outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Periodic lateralized epileptiform discharges -- long-term outcome in adults .
	manualset3
244639	3	422224	7	NULL	NULL	0	NULL	adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Periodic lateralized epileptiform discharges -- long-term outcome in adults .
	manualset3
244640	1	422225	7	NULL	NULL	0	NULL	systematic survey	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	An extensive and systematic survey has been undertaken to evaluate the contamination with PAHs of urban soils in Beijing , China .
	manualset3
244641	2	422225	7	NULL	NULL	0	NULL	contamination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An extensive and systematic survey has been undertaken to evaluate the contamination with PAHs of urban soils in Beijing , China .
	manualset3
244642	3	422225	7	NULL	NULL	0	NULL	PAHs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An extensive and systematic survey has been undertaken to evaluate the contamination with PAHs of urban soils in Beijing , China .
	manualset3
244643	4	422225	7	NULL	NULL	NULL	NULL	urban soils	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An extensive and systematic survey has been undertaken to evaluate the contamination with PAHs of urban soils in Beijing , China .
	manualset3
244644	5	422225	7	NULL	NULL	0	NULL	Beijing	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	An extensive and systematic survey has been undertaken to evaluate the contamination with PAHs of urban soils in Beijing , China .
	manualset3
244645	6	422225	7	NULL	NULL	0	NULL	China	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	An extensive and systematic survey has been undertaken to evaluate the contamination with PAHs of urban soils in Beijing , China .
	manualset3
244646	1	422226	7	NULL	NULL	0	NULL	IGF-II mRNA expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	IGF-II mRNA expression in breast cancer : predictive value and relationship to other prognostic factors .
	manualset3
244647	2	422226	7	NULL	NULL	0	NULL	breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	IGF-II mRNA expression in breast cancer : predictive value and relationship to other prognostic factors .
	manualset3
244648	3	422226	7	NULL	NULL	0	NULL	predictive value	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	IGF-II mRNA expression in breast cancer : predictive value and relationship to other prognostic factors .
	manualset3
244649	4	422226	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	IGF-II mRNA expression in breast cancer : predictive value and relationship to other prognostic factors .
	manualset3
244650	5	422226	7	NULL	NULL	0	NULL	prognostic factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	IGF-II mRNA expression in breast cancer : predictive value and relationship to other prognostic factors .
	manualset3
244651	1	422227	7	NULL	NULL	0	NULL	1918	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1918 , the worst influenza pandemic on record caused 675 , 000 deaths in the United States and up to 40 million deaths worldwide .
	manualset3
244652	2	422227	7	NULL	NULL	0	NULL	worst influenza pandemic	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1918 , the worst influenza pandemic on record caused 675 , 000 deaths in the United States and up to 40 million deaths worldwide .
	manualset3
244653	3	422227	7	NULL	NULL	0	NULL	 record	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1918 , the worst influenza pandemic on record caused 675 , 000 deaths in the United States and up to 40 million deaths worldwide .
	manualset3
244654	4	422227	7	NULL	NULL	0	NULL	675 , 000 deaths	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1918 , the worst influenza pandemic on record caused 675 , 000 deaths in the United States and up to 40 million deaths worldwide .
	manualset3
244655	5	422227	7	NULL	NULL	0	NULL	United States	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1918 , the worst influenza pandemic on record caused 675 , 000 deaths in the United States and up to 40 million deaths worldwide .
	manualset3
244656	6	422227	7	NULL	NULL	0	NULL	40 million deaths worldwide	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	In 1918 , the worst influenza pandemic on record caused 675 , 000 deaths in the United States and up to 40 million deaths worldwide .
	manualset3
244657	1	422228	7	NULL	NULL	0	NULL	Inherited retinal degeneration	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Inherited retinal degeneration affects about 1 in 2 , 000-3 , 000 individuals in the world and is the leading cause of visual loss in young people and accounts for a large proportion of blindness in adult life .
	manualset3
244658	2	422228	7	NULL	NULL	0	NULL	 1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Inherited retinal degeneration affects about 1 in 2 , 000-3 , 000 individuals in the world and is the leading cause of visual loss in young people and accounts for a large proportion of blindness in adult life .
	manualset3
244659	3	422228	7	NULL	NULL	0	NULL	 2 , 000 individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Inherited retinal degeneration affects about 1 in 2 , 000-3 , 000 individuals in the world and is the leading cause of visual loss in young people and accounts for a large proportion of blindness in adult life .
	manualset3
244660	4	422228	7	NULL	NULL	0	NULL	3 , 000 individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Inherited retinal degeneration affects about 1 in 2 , 000-3 , 000 individuals in the world and is the leading cause of visual loss in young people and accounts for a large proportion of blindness in adult life .
	manualset3
244661	5	422228	7	NULL	NULL	0	NULL	 world	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Inherited retinal degeneration affects about 1 in 2 , 000-3 , 000 individuals in the world and is the leading cause of visual loss in young people and accounts for a large proportion of blindness in adult life .
	manualset3
244662	6	422228	7	NULL	NULL	0	NULL	 leading cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inherited retinal degeneration affects about 1 in 2 , 000-3 , 000 individuals in the world and is the leading cause of visual loss in young people and accounts for a large proportion of blindness in adult life .
	manualset3
244663	7	422228	7	NULL	NULL	0	NULL	visual loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inherited retinal degeneration affects about 1 in 2 , 000-3 , 000 individuals in the world and is the leading cause of visual loss in young people and accounts for a large proportion of blindness in adult life .
	manualset3
244664	8	422228	7	NULL	NULL	0	NULL	young people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Inherited retinal degeneration affects about 1 in 2 , 000-3 , 000 individuals in the world and is the leading cause of visual loss in young people and accounts for a large proportion of blindness in adult life .
	manualset3
244665	9	422228	7	NULL	NULL	0	NULL	 large proportion	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Inherited retinal degeneration affects about 1 in 2 , 000-3 , 000 individuals in the world and is the leading cause of visual loss in young people and accounts for a large proportion of blindness in adult life .
	manualset3
244666	10	422228	7	NULL	NULL	0	NULL	blindness 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Inherited retinal degeneration affects about 1 in 2 , 000-3 , 000 individuals in the world and is the leading cause of visual loss in young people and accounts for a large proportion of blindness in adult life .
	manualset3
244667	11	422228	7	NULL	NULL	0	NULL	adult life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inherited retinal degeneration affects about 1 in 2 , 000-3 , 000 individuals in the world and is the leading cause of visual loss in young people and accounts for a large proportion of blindness in adult life .
	manualset3
244668	1	422229	7	NULL	NULL	0	NULL	Interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions of radiolabeled tuftsin with human neutrophils .
	manualset3
244669	2	422229	7	NULL	NULL	0	NULL	radiolabeled tuftsin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions of radiolabeled tuftsin with human neutrophils .
	manualset3
244670	3	422229	7	NULL	NULL	0	NULL	human neutrophils	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Interactions of radiolabeled tuftsin with human neutrophils .
	manualset3
244671	1	422230	7	NULL	NULL	0	NULL	Hand-held echocardiography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Hand-held echocardiography with Doppler capability for the assessment of critically-ill patients : is it reliable ?
	manualset3
244672	2	422230	7	NULL	NULL	0	NULL	Doppler capability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Hand-held echocardiography with Doppler capability for the assessment of critically-ill patients : is it reliable ?
	manualset3
244673	3	422230	7	NULL	NULL	0	NULL	assessment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hand-held echocardiography with Doppler capability for the assessment of critically-ill patients : is it reliable ?
	manualset3
244674	4	422230	7	NULL	NULL	0	NULL	critically-ill patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Hand-held echocardiography with Doppler capability for the assessment of critically-ill patients : is it reliable ?
	manualset3
244697	1	422231	7	NULL	NULL	0	NULL	nine risk factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The following nine risk factors , which may significantly influence the relationship between the time required for defervescence and the duration of neutropenia - age ; hematological diseases ; the leukocyte count during the febrile period ; the reduction in leukocyte count per day before the onset of FN ; the prophylactic administration of antimycotic agents ; sterilization of the intestinal tract ; and urine albumin content , creatine level , and C-reactive protein ( CRP ) level - were expressed in points and their sum was termed risk points .
	manualset3
244698	2	422231	7	NULL	NULL	0	NULL	 relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The following nine risk factors , which may significantly influence the relationship between the time required for defervescence and the duration of neutropenia - age ; hematological diseases ; the leukocyte count during the febrile period ; the reduction in leukocyte count per day before the onset of FN ; the prophylactic administration of antimycotic agents ; sterilization of the intestinal tract ; and urine albumin content , creatine level , and C-reactive protein ( CRP ) level - were expressed in points and their sum was termed risk points .
	manualset3
244699	3	422231	7	NULL	NULL	0	NULL	 time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	The following nine risk factors , which may significantly influence the relationship between the time required for defervescence and the duration of neutropenia - age ; hematological diseases ; the leukocyte count during the febrile period ; the reduction in leukocyte count per day before the onset of FN ; the prophylactic administration of antimycotic agents ; sterilization of the intestinal tract ; and urine albumin content , creatine level , and C-reactive protein ( CRP ) level - were expressed in points and their sum was termed risk points .
	manualset3
244700	4	422231	7	NULL	NULL	0	NULL	defervescence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The following nine risk factors , which may significantly influence the relationship between the time required for defervescence and the duration of neutropenia - age ; hematological diseases ; the leukocyte count during the febrile period ; the reduction in leukocyte count per day before the onset of FN ; the prophylactic administration of antimycotic agents ; sterilization of the intestinal tract ; and urine albumin content , creatine level , and C-reactive protein ( CRP ) level - were expressed in points and their sum was termed risk points .
	manualset3
244701	5	422231	7	NULL	NULL	0	NULL	duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The following nine risk factors , which may significantly influence the relationship between the time required for defervescence and the duration of neutropenia - age ; hematological diseases ; the leukocyte count during the febrile period ; the reduction in leukocyte count per day before the onset of FN ; the prophylactic administration of antimycotic agents ; sterilization of the intestinal tract ; and urine albumin content , creatine level , and C-reactive protein ( CRP ) level - were expressed in points and their sum was termed risk points .
	manualset3
244702	6	422231	7	NULL	NULL	0	NULL	 neutropenia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The following nine risk factors , which may significantly influence the relationship between the time required for defervescence and the duration of neutropenia - age ; hematological diseases ; the leukocyte count during the febrile period ; the reduction in leukocyte count per day before the onset of FN ; the prophylactic administration of antimycotic agents ; sterilization of the intestinal tract ; and urine albumin content , creatine level , and C-reactive protein ( CRP ) level - were expressed in points and their sum was termed risk points .
	manualset3
244703	7	422231	7	NULL	NULL	0	NULL	age	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The following nine risk factors , which may significantly influence the relationship between the time required for defervescence and the duration of neutropenia - age ; hematological diseases ; the leukocyte count during the febrile period ; the reduction in leukocyte count per day before the onset of FN ; the prophylactic administration of antimycotic agents ; sterilization of the intestinal tract ; and urine albumin content , creatine level , and C-reactive protein ( CRP ) level - were expressed in points and their sum was termed risk points .
	manualset3
244704	8	422231	7	NULL	NULL	0	NULL	hematological diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The following nine risk factors , which may significantly influence the relationship between the time required for defervescence and the duration of neutropenia - age ; hematological diseases ; the leukocyte count during the febrile period ; the reduction in leukocyte count per day before the onset of FN ; the prophylactic administration of antimycotic agents ; sterilization of the intestinal tract ; and urine albumin content , creatine level , and C-reactive protein ( CRP ) level - were expressed in points and their sum was termed risk points .
	manualset3
244705	9	422231	7	NULL	NULL	0	NULL	leukocyte count 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The following nine risk factors , which may significantly influence the relationship between the time required for defervescence and the duration of neutropenia - age ; hematological diseases ; the leukocyte count during the febrile period ; the reduction in leukocyte count per day before the onset of FN ; the prophylactic administration of antimycotic agents ; sterilization of the intestinal tract ; and urine albumin content , creatine level , and C-reactive protein ( CRP ) level - were expressed in points and their sum was termed risk points .
	manualset3
244706	10	422231	7	NULL	NULL	0	NULL	febrile period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The following nine risk factors , which may significantly influence the relationship between the time required for defervescence and the duration of neutropenia - age ; hematological diseases ; the leukocyte count during the febrile period ; the reduction in leukocyte count per day before the onset of FN ; the prophylactic administration of antimycotic agents ; sterilization of the intestinal tract ; and urine albumin content , creatine level , and C-reactive protein ( CRP ) level - were expressed in points and their sum was termed risk points .
	manualset3
244707	11	422231	7	NULL	NULL	0	NULL	reduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The following nine risk factors , which may significantly influence the relationship between the time required for defervescence and the duration of neutropenia - age ; hematological diseases ; the leukocyte count during the febrile period ; the reduction in leukocyte count per day before the onset of FN ; the prophylactic administration of antimycotic agents ; sterilization of the intestinal tract ; and urine albumin content , creatine level , and C-reactive protein ( CRP ) level - were expressed in points and their sum was termed risk points .
	manualset3
244708	12	422231	7	NULL	NULL	0	NULL	leukocyte count per day	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The following nine risk factors , which may significantly influence the relationship between the time required for defervescence and the duration of neutropenia - age ; hematological diseases ; the leukocyte count during the febrile period ; the reduction in leukocyte count per day before the onset of FN ; the prophylactic administration of antimycotic agents ; sterilization of the intestinal tract ; and urine albumin content , creatine level , and C-reactive protein ( CRP ) level - were expressed in points and their sum was termed risk points .
	manualset3
244709	13	422231	7	NULL	NULL	0	NULL	onset	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The following nine risk factors , which may significantly influence the relationship between the time required for defervescence and the duration of neutropenia - age ; hematological diseases ; the leukocyte count during the febrile period ; the reduction in leukocyte count per day before the onset of FN ; the prophylactic administration of antimycotic agents ; sterilization of the intestinal tract ; and urine albumin content , creatine level , and C-reactive protein ( CRP ) level - were expressed in points and their sum was termed risk points .
	manualset3
244710	14	422231	7	NULL	NULL	0	NULL	FN	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The following nine risk factors , which may significantly influence the relationship between the time required for defervescence and the duration of neutropenia - age ; hematological diseases ; the leukocyte count during the febrile period ; the reduction in leukocyte count per day before the onset of FN ; the prophylactic administration of antimycotic agents ; sterilization of the intestinal tract ; and urine albumin content , creatine level , and C-reactive protein ( CRP ) level - were expressed in points and their sum was termed risk points .
	manualset3
244711	15	422231	7	NULL	NULL	0	NULL	prophylactic administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The following nine risk factors , which may significantly influence the relationship between the time required for defervescence and the duration of neutropenia - age ; hematological diseases ; the leukocyte count during the febrile period ; the reduction in leukocyte count per day before the onset of FN ; the prophylactic administration of antimycotic agents ; sterilization of the intestinal tract ; and urine albumin content , creatine level , and C-reactive protein ( CRP ) level - were expressed in points and their sum was termed risk points .
	manualset3
244712	16	422231	7	NULL	NULL	0	NULL	antimycotic agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The following nine risk factors , which may significantly influence the relationship between the time required for defervescence and the duration of neutropenia - age ; hematological diseases ; the leukocyte count during the febrile period ; the reduction in leukocyte count per day before the onset of FN ; the prophylactic administration of antimycotic agents ; sterilization of the intestinal tract ; and urine albumin content , creatine level , and C-reactive protein ( CRP ) level - were expressed in points and their sum was termed risk points .
	manualset3
244713	17	422231	7	NULL	NULL	0	NULL	sterilization 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The following nine risk factors , which may significantly influence the relationship between the time required for defervescence and the duration of neutropenia - age ; hematological diseases ; the leukocyte count during the febrile period ; the reduction in leukocyte count per day before the onset of FN ; the prophylactic administration of antimycotic agents ; sterilization of the intestinal tract ; and urine albumin content , creatine level , and C-reactive protein ( CRP ) level - were expressed in points and their sum was termed risk points .
	manualset3
244714	18	422231	7	NULL	NULL	0	NULL	 intestinal tract 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The following nine risk factors , which may significantly influence the relationship between the time required for defervescence and the duration of neutropenia - age ; hematological diseases ; the leukocyte count during the febrile period ; the reduction in leukocyte count per day before the onset of FN ; the prophylactic administration of antimycotic agents ; sterilization of the intestinal tract ; and urine albumin content , creatine level , and C-reactive protein ( CRP ) level - were expressed in points and their sum was termed risk points .
	manualset3
244715	19	422231	7	NULL	NULL	0	NULL	urine albumin content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The following nine risk factors , which may significantly influence the relationship between the time required for defervescence and the duration of neutropenia - age ; hematological diseases ; the leukocyte count during the febrile period ; the reduction in leukocyte count per day before the onset of FN ; the prophylactic administration of antimycotic agents ; sterilization of the intestinal tract ; and urine albumin content , creatine level , and C-reactive protein ( CRP ) level - were expressed in points and their sum was termed risk points .
	manualset3
244716	20	422231	7	NULL	NULL	0	NULL	creatine level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The following nine risk factors , which may significantly influence the relationship between the time required for defervescence and the duration of neutropenia - age ; hematological diseases ; the leukocyte count during the febrile period ; the reduction in leukocyte count per day before the onset of FN ; the prophylactic administration of antimycotic agents ; sterilization of the intestinal tract ; and urine albumin content , creatine level , and C-reactive protein ( CRP ) level - were expressed in points and their sum was termed risk points .
	manualset3
244717	21	422231	7	NULL	NULL	0	NULL	 C-reactive protein ( CRP ) level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The following nine risk factors , which may significantly influence the relationship between the time required for defervescence and the duration of neutropenia - age ; hematological diseases ; the leukocyte count during the febrile period ; the reduction in leukocyte count per day before the onset of FN ; the prophylactic administration of antimycotic agents ; sterilization of the intestinal tract ; and urine albumin content , creatine level , and C-reactive protein ( CRP ) level - were expressed in points and their sum was termed risk points .
	manualset3
244718	22	422231	7	NULL	NULL	0	NULL	 points	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The following nine risk factors , which may significantly influence the relationship between the time required for defervescence and the duration of neutropenia - age ; hematological diseases ; the leukocyte count during the febrile period ; the reduction in leukocyte count per day before the onset of FN ; the prophylactic administration of antimycotic agents ; sterilization of the intestinal tract ; and urine albumin content , creatine level , and C-reactive protein ( CRP ) level - were expressed in points and their sum was termed risk points .
	manualset3
244719	23	422231	7	NULL	NULL	0	NULL	sum	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The following nine risk factors , which may significantly influence the relationship between the time required for defervescence and the duration of neutropenia - age ; hematological diseases ; the leukocyte count during the febrile period ; the reduction in leukocyte count per day before the onset of FN ; the prophylactic administration of antimycotic agents ; sterilization of the intestinal tract ; and urine albumin content , creatine level , and C-reactive protein ( CRP ) level - were expressed in points and their sum was termed risk points .
	manualset3
244720	24	422231	7	NULL	NULL	0	NULL	risk points	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The following nine risk factors , which may significantly influence the relationship between the time required for defervescence and the duration of neutropenia - age ; hematological diseases ; the leukocyte count during the febrile period ; the reduction in leukocyte count per day before the onset of FN ; the prophylactic administration of antimycotic agents ; sterilization of the intestinal tract ; and urine albumin content , creatine level , and C-reactive protein ( CRP ) level - were expressed in points and their sum was termed risk points .
	manualset3
244721	1	422232	7	NULL	NULL	0	NULL	external loading apparatus	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	An external loading apparatus was applied for 8 days , and growth was measured as the distance between fluorescent markers administered 24 and 48 h prior to euthanasia .
	manualset3
244722	2	422232	7	NULL	NULL	0	NULL	8 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	An external loading apparatus was applied for 8 days , and growth was measured as the distance between fluorescent markers administered 24 and 48 h prior to euthanasia .
	manualset3
244723	3	422232	7	NULL	NULL	0	NULL	growth	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An external loading apparatus was applied for 8 days , and growth was measured as the distance between fluorescent markers administered 24 and 48 h prior to euthanasia .
	manualset3
244724	4	422232	7	NULL	NULL	0	NULL	distance	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An external loading apparatus was applied for 8 days , and growth was measured as the distance between fluorescent markers administered 24 and 48 h prior to euthanasia .
	manualset3
244725	5	422232	7	NULL	NULL	0	NULL	 fluorescent markers 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	An external loading apparatus was applied for 8 days , and growth was measured as the distance between fluorescent markers administered 24 and 48 h prior to euthanasia .
	manualset3
244726	6	422232	7	NULL	NULL	NULL	NULL	24 h	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An external loading apparatus was applied for 8 days , and growth was measured as the distance between fluorescent markers administered 24 and 48 h prior to euthanasia .
	manualset3
244727	7	422232	7	NULL	NULL	NULL	NULL	48 h	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An external loading apparatus was applied for 8 days , and growth was measured as the distance between fluorescent markers administered 24 and 48 h prior to euthanasia .
	manualset3
244728	8	422232	7	NULL	NULL	0	NULL	euthanasia	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	An external loading apparatus was applied for 8 days , and growth was measured as the distance between fluorescent markers administered 24 and 48 h prior to euthanasia .
	manualset3
244729	1	422233	7	NULL	NULL	0	NULL	 conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Those conditions lead to an accumulation of bile acids in the cord blood serum , meconium and amniotic fluid that may account for a diminished fetal well-being and sudden intra-uterine death by ICP .
	manualset3
244730	2	422233	7	NULL	NULL	0	NULL	accumulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Those conditions lead to an accumulation of bile acids in the cord blood serum , meconium and amniotic fluid that may account for a diminished fetal well-being and sudden intra-uterine death by ICP .
	manualset3
244731	3	422233	7	NULL	NULL	0	NULL	bile acids	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Those conditions lead to an accumulation of bile acids in the cord blood serum , meconium and amniotic fluid that may account for a diminished fetal well-being and sudden intra-uterine death by ICP .
	manualset3
244732	4	422233	7	NULL	NULL	0	NULL	cord blood serum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Those conditions lead to an accumulation of bile acids in the cord blood serum , meconium and amniotic fluid that may account for a diminished fetal well-being and sudden intra-uterine death by ICP .
	manualset3
244733	5	422233	7	NULL	NULL	0	NULL	meconium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Those conditions lead to an accumulation of bile acids in the cord blood serum , meconium and amniotic fluid that may account for a diminished fetal well-being and sudden intra-uterine death by ICP .
	manualset3
244734	6	422233	7	NULL	NULL	0	NULL	amniotic fluid	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Those conditions lead to an accumulation of bile acids in the cord blood serum , meconium and amniotic fluid that may account for a diminished fetal well-being and sudden intra-uterine death by ICP .
	manualset3
244735	7	422233	7	NULL	NULL	0	NULL	diminished fetal well-being	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Those conditions lead to an accumulation of bile acids in the cord blood serum , meconium and amniotic fluid that may account for a diminished fetal well-being and sudden intra-uterine death by ICP .
	manualset3
244736	8	422233	7	NULL	NULL	0	NULL	 sudden intra-uterine death 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Those conditions lead to an accumulation of bile acids in the cord blood serum , meconium and amniotic fluid that may account for a diminished fetal well-being and sudden intra-uterine death by ICP .
	manualset3
244737	9	422233	7	NULL	NULL	0	NULL	ICP	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Those conditions lead to an accumulation of bile acids in the cord blood serum , meconium and amniotic fluid that may account for a diminished fetal well-being and sudden intra-uterine death by ICP .
	manualset3
244738	1	422234	7	NULL	NULL	NULL	NULL	Primary lingual abscess	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Primary lingual abscess presenting as acute swelling of the tongue obstructing the upper airway : diagnosis with MR .
	manualset3
244739	2	422234	7	NULL	NULL	0	NULL	acute swelling	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary lingual abscess presenting as acute swelling of the tongue obstructing the upper airway : diagnosis with MR .
	manualset3
244740	3	422234	7	NULL	NULL	0	NULL	tongue	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary lingual abscess presenting as acute swelling of the tongue obstructing the upper airway : diagnosis with MR .
	manualset3
244741	4	422234	7	NULL	NULL	0	NULL	 upper airway	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary lingual abscess presenting as acute swelling of the tongue obstructing the upper airway : diagnosis with MR .
	manualset3
244742	5	422234	7	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary lingual abscess presenting as acute swelling of the tongue obstructing the upper airway : diagnosis with MR .
	manualset3
244743	6	422234	7	NULL	NULL	0	NULL	MR	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Primary lingual abscess presenting as acute swelling of the tongue obstructing the upper airway : diagnosis with MR .
	manualset3
244744	1	422235	7	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevailing hypothesis is that high-LET radiations induce DNA double strand-breaks ( DSB ) that are more complex and clustered , and are thereby more challenging to repair .
	manualset3
244745	2	422235	7	NULL	NULL	0	NULL	high-LET radiations	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevailing hypothesis is that high-LET radiations induce DNA double strand-breaks ( DSB ) that are more complex and clustered , and are thereby more challenging to repair .
	manualset3
244746	3	422235	7	NULL	NULL	0	NULL	DNA double strand-breaks ( DSB )	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevailing hypothesis is that high-LET radiations induce DNA double strand-breaks ( DSB ) that are more complex and clustered , and are thereby more challenging to repair .
	manualset3
244747	4	422235	7	NULL	NULL	0	NULL	repair	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The prevailing hypothesis is that high-LET radiations induce DNA double strand-breaks ( DSB ) that are more complex and clustered , and are thereby more challenging to repair .
	manualset3
244748	1	422236	7	NULL	NULL	0	NULL	TRAINING PROGRAM	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A TRAINING PROGRAM IN BLOOD BANKING FOR MEDICAL TECHNOLOGISTS .
	manualset3
244749	2	422236	7	NULL	NULL	0	NULL	BLOOD BANKING	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A TRAINING PROGRAM IN BLOOD BANKING FOR MEDICAL TECHNOLOGISTS .
	manualset3
244750	3	422236	7	NULL	NULL	0	NULL	MEDICAL TECHNOLOGISTS	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A TRAINING PROGRAM IN BLOOD BANKING FOR MEDICAL TECHNOLOGISTS .
	manualset3
244751	1	422237	7	NULL	NULL	0	NULL	recent discovery 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent discovery and cloning of the first mammalian clock gene is expected to lead to rapid advances in the understanding of the genetic and molecular mechanisms underlying circadian rhythmicity in mammals .
	manualset3
244752	2	422237	7	NULL	NULL	0	NULL	cloning 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent discovery and cloning of the first mammalian clock gene is expected to lead to rapid advances in the understanding of the genetic and molecular mechanisms underlying circadian rhythmicity in mammals .
	manualset3
244753	3	422237	7	NULL	NULL	0	NULL	first mammalian clock gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent discovery and cloning of the first mammalian clock gene is expected to lead to rapid advances in the understanding of the genetic and molecular mechanisms underlying circadian rhythmicity in mammals .
	manualset3
244754	4	422237	7	NULL	NULL	0	NULL	advances	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent discovery and cloning of the first mammalian clock gene is expected to lead to rapid advances in the understanding of the genetic and molecular mechanisms underlying circadian rhythmicity in mammals .
	manualset3
244755	5	422237	7	NULL	NULL	0	NULL	understanding 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent discovery and cloning of the first mammalian clock gene is expected to lead to rapid advances in the understanding of the genetic and molecular mechanisms underlying circadian rhythmicity in mammals .
	manualset3
244756	6	422237	7	NULL	NULL	0	NULL	genetic mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent discovery and cloning of the first mammalian clock gene is expected to lead to rapid advances in the understanding of the genetic and molecular mechanisms underlying circadian rhythmicity in mammals .
	manualset3
244757	7	422237	7	NULL	NULL	0	NULL	molecular mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent discovery and cloning of the first mammalian clock gene is expected to lead to rapid advances in the understanding of the genetic and molecular mechanisms underlying circadian rhythmicity in mammals .
	manualset3
244758	8	422237	7	NULL	NULL	0	NULL	circadian rhythmicity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent discovery and cloning of the first mammalian clock gene is expected to lead to rapid advances in the understanding of the genetic and molecular mechanisms underlying circadian rhythmicity in mammals .
	manualset3
244759	9	422237	7	NULL	NULL	0	NULL	mammals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The recent discovery and cloning of the first mammalian clock gene is expected to lead to rapid advances in the understanding of the genetic and molecular mechanisms underlying circadian rhythmicity in mammals .
	manualset3
244760	1	422238	7	NULL	NULL	0	NULL	PucM structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The PucM structure determined for the TRP family leads to the conclusion that diverse members of the TRP family would function similarly to PucM as HIU hydrolase .
	manualset3
244761	2	422238	7	NULL	NULL	0	NULL	TRP family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The PucM structure determined for the TRP family leads to the conclusion that diverse members of the TRP family would function similarly to PucM as HIU hydrolase .
	manualset3
244762	3	422238	7	NULL	NULL	0	NULL	conclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The PucM structure determined for the TRP family leads to the conclusion that diverse members of the TRP family would function similarly to PucM as HIU hydrolase .
	manualset3
244763	4	422238	7	NULL	NULL	0	NULL	diverse members	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The PucM structure determined for the TRP family leads to the conclusion that diverse members of the TRP family would function similarly to PucM as HIU hydrolase .
	manualset3
244764	5	422238	7	NULL	NULL	0	NULL	TRP family	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The PucM structure determined for the TRP family leads to the conclusion that diverse members of the TRP family would function similarly to PucM as HIU hydrolase .
	manualset3
244765	6	422238	7	NULL	NULL	0	NULL	PucM	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The PucM structure determined for the TRP family leads to the conclusion that diverse members of the TRP family would function similarly to PucM as HIU hydrolase .
	manualset3
244766	7	422238	7	NULL	NULL	0	NULL	HIU hydrolase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The PucM structure determined for the TRP family leads to the conclusion that diverse members of the TRP family would function similarly to PucM as HIU hydrolase .
	manualset3
244767	1	422239	7	NULL	NULL	0	NULL	 Splitting 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Splitting of supplemental revenues in intensive care medicine ) .
	manualset3
244768	2	422239	7	NULL	NULL	0	NULL	 supplemental revenues	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Splitting of supplemental revenues in intensive care medicine ) .
	manualset3
244769	3	422239	7	NULL	NULL	0	NULL	intensive care medicine	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Splitting of supplemental revenues in intensive care medicine ) .
	manualset3
244770	1	422240	7	NULL	NULL	0	NULL	oscillations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	During these oscillations , the telomeres are clustered at the spindle pole body ( SPB ) , located at the leading edge of the moving nucleus and the rest of each chromosome dangles behind .
	manualset3
244771	2	422240	7	NULL	NULL	NULL	NULL	telomeres	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During these oscillations , the telomeres are clustered at the spindle pole body ( SPB ) , located at the leading edge of the moving nucleus and the rest of each chromosome dangles behind .
	manualset3
244772	3	422240	7	NULL	NULL	0	NULL	spindle pole body ( SPB )	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	During these oscillations , the telomeres are clustered at the spindle pole body ( SPB ) , located at the leading edge of the moving nucleus and the rest of each chromosome dangles behind .
	manualset3
244773	4	422240	7	NULL	NULL	0	NULL	moving nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	During these oscillations , the telomeres are clustered at the spindle pole body ( SPB ) , located at the leading edge of the moving nucleus and the rest of each chromosome dangles behind .
	manualset3
244774	5	422240	7	NULL	NULL	0	NULL	chromosome	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	During these oscillations , the telomeres are clustered at the spindle pole body ( SPB ) , located at the leading edge of the moving nucleus and the rest of each chromosome dangles behind .
	manualset3
244775	6	422240	7	NULL	NULL	0	NULL	leading edge	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	During these oscillations , the telomeres are clustered at the spindle pole body ( SPB ) , located at the leading edge of the moving nucleus and the rest of each chromosome dangles behind .
	manualset3
244776	1	422241	7	NULL	NULL	0	NULL	external stimulus	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	An external stimulus that mimics Mls locus responses .
	manualset3
244777	2	422241	7	NULL	NULL	0	NULL	Mls locus responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An external stimulus that mimics Mls locus responses .
	manualset3
244778	1	422242	7	NULL	NULL	0	NULL	different clinical phenotypes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The different clinical phenotypes associated with the different HPS frameshifts we observed suggests that differentially truncated HPS polypeptides may have somewhat different consequences for subcellular function .
	manualset3
244779	2	422242	7	NULL	NULL	0	NULL	different HPS frameshifts	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The different clinical phenotypes associated with the different HPS frameshifts we observed suggests that differentially truncated HPS polypeptides may have somewhat different consequences for subcellular function .
	manualset3
244780	3	422242	7	NULL	NULL	0	NULL	differentially truncated HPS polypeptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	The different clinical phenotypes associated with the different HPS frameshifts we observed suggests that differentially truncated HPS polypeptides may have somewhat different consequences for subcellular function .
	manualset3
244781	4	422242	7	NULL	NULL	0	NULL	subcellular function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The different clinical phenotypes associated with the different HPS frameshifts we observed suggests that differentially truncated HPS polypeptides may have somewhat different consequences for subcellular function .
	manualset3
244782	1	422243	7	NULL	NULL	0	NULL	result 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The result indicated that the primers can be used as molecular tool for future field survey of Salmonella both in food and in clinical specimens .
	manualset3
244783	2	422243	7	NULL	NULL	0	NULL	 primers	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	The result indicated that the primers can be used as molecular tool for future field survey of Salmonella both in food and in clinical specimens .
	manualset3
244784	3	422243	7	NULL	NULL	0	NULL	molecular tool	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The result indicated that the primers can be used as molecular tool for future field survey of Salmonella both in food and in clinical specimens .
	manualset3
244785	4	422243	7	NULL	NULL	0	NULL	future field survey	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The result indicated that the primers can be used as molecular tool for future field survey of Salmonella both in food and in clinical specimens .
	manualset3
244786	5	422243	7	NULL	NULL	0	NULL	Salmonella 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The result indicated that the primers can be used as molecular tool for future field survey of Salmonella both in food and in clinical specimens .
	manualset3
244787	6	422243	7	NULL	NULL	0	NULL	 food	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	The result indicated that the primers can be used as molecular tool for future field survey of Salmonella both in food and in clinical specimens .
	manualset3
244788	7	422243	7	NULL	NULL	0	NULL	clinical specimens	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The result indicated that the primers can be used as molecular tool for future field survey of Salmonella both in food and in clinical specimens .
	manualset3
244789	1	422244	7	NULL	NULL	0	NULL	hybrid taxa	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	This is particularly true for hybrid taxa , where differential introgression of genome parts leads to incongruity between data sets .
	manualset3
244790	2	422244	7	NULL	NULL	0	NULL	differential introgression	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This is particularly true for hybrid taxa , where differential introgression of genome parts leads to incongruity between data sets .
	manualset3
244791	3	422244	7	NULL	NULL	NULL	NULL	genome parts	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This is particularly true for hybrid taxa , where differential introgression of genome parts leads to incongruity between data sets .
	manualset3
244792	4	422244	7	NULL	NULL	0	NULL	data sets 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This is particularly true for hybrid taxa , where differential introgression of genome parts leads to incongruity between data sets .
	manualset3
244793	1	422245	7	NULL	NULL	0	NULL	relative retention times 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative retention times and elution order of each reduced metabolite are different with each solvent system and hence help confirm the identities of Ring-A reduced metabolites made in vivo from physiological quantities of ( 3H ) aldosterone .
	manualset3
244794	2	422245	7	NULL	NULL	0	NULL	elution order 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative retention times and elution order of each reduced metabolite are different with each solvent system and hence help confirm the identities of Ring-A reduced metabolites made in vivo from physiological quantities of ( 3H ) aldosterone .
	manualset3
244795	3	422245	7	NULL	NULL	0	NULL	reduced metabolite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative retention times and elution order of each reduced metabolite are different with each solvent system and hence help confirm the identities of Ring-A reduced metabolites made in vivo from physiological quantities of ( 3H ) aldosterone .
	manualset3
244796	4	422245	7	NULL	NULL	0	NULL	solvent system	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative retention times and elution order of each reduced metabolite are different with each solvent system and hence help confirm the identities of Ring-A reduced metabolites made in vivo from physiological quantities of ( 3H ) aldosterone .
	manualset3
244797	5	422245	7	NULL	NULL	0	NULL	 identities 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative retention times and elution order of each reduced metabolite are different with each solvent system and hence help confirm the identities of Ring-A reduced metabolites made in vivo from physiological quantities of ( 3H ) aldosterone .
	manualset3
244798	6	422245	7	NULL	NULL	0	NULL	Ring-A reduced metabolites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative retention times and elution order of each reduced metabolite are different with each solvent system and hence help confirm the identities of Ring-A reduced metabolites made in vivo from physiological quantities of ( 3H ) aldosterone .
	manualset3
244799	7	422245	7	NULL	NULL	0	NULL	physiological quantities 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative retention times and elution order of each reduced metabolite are different with each solvent system and hence help confirm the identities of Ring-A reduced metabolites made in vivo from physiological quantities of ( 3H ) aldosterone .
	manualset3
244800	8	422245	7	NULL	NULL	0	NULL	( 3H ) aldosterone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The relative retention times and elution order of each reduced metabolite are different with each solvent system and hence help confirm the identities of Ring-A reduced metabolites made in vivo from physiological quantities of ( 3H ) aldosterone .
	manualset3
244801	1	422246	7	NULL	NULL	0	NULL	 authors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors evaluated the effect of four types of data manipulation : ( a ) reconstruction of data with different convolution filters ( target reconstruction ) , ( b ) extension of the range of CT numbers , ( c ) mathematical filtration to enhance edges , and ( d ) correction for beam hardening .
	manualset3
244802	2	422246	7	NULL	NULL	0	NULL	 effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors evaluated the effect of four types of data manipulation : ( a ) reconstruction of data with different convolution filters ( target reconstruction ) , ( b ) extension of the range of CT numbers , ( c ) mathematical filtration to enhance edges , and ( d ) correction for beam hardening .
	manualset3
244803	3	422246	7	NULL	NULL	0	NULL	four types	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors evaluated the effect of four types of data manipulation : ( a ) reconstruction of data with different convolution filters ( target reconstruction ) , ( b ) extension of the range of CT numbers , ( c ) mathematical filtration to enhance edges , and ( d ) correction for beam hardening .
	manualset3
244804	4	422246	7	NULL	NULL	0	NULL	data manipulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors evaluated the effect of four types of data manipulation : ( a ) reconstruction of data with different convolution filters ( target reconstruction ) , ( b ) extension of the range of CT numbers , ( c ) mathematical filtration to enhance edges , and ( d ) correction for beam hardening .
	manualset3
244805	5	422246	7	NULL	NULL	0	NULL	reconstruction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors evaluated the effect of four types of data manipulation : ( a ) reconstruction of data with different convolution filters ( target reconstruction ) , ( b ) extension of the range of CT numbers , ( c ) mathematical filtration to enhance edges , and ( d ) correction for beam hardening .
	manualset3
244806	6	422246	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors evaluated the effect of four types of data manipulation : ( a ) reconstruction of data with different convolution filters ( target reconstruction ) , ( b ) extension of the range of CT numbers , ( c ) mathematical filtration to enhance edges , and ( d ) correction for beam hardening .
	manualset3
244807	7	422246	7	NULL	NULL	0	NULL	different convolution filters	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors evaluated the effect of four types of data manipulation : ( a ) reconstruction of data with different convolution filters ( target reconstruction ) , ( b ) extension of the range of CT numbers , ( c ) mathematical filtration to enhance edges , and ( d ) correction for beam hardening .
	manualset3
244808	8	422246	7	NULL	NULL	0	NULL	target reconstruction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors evaluated the effect of four types of data manipulation : ( a ) reconstruction of data with different convolution filters ( target reconstruction ) , ( b ) extension of the range of CT numbers , ( c ) mathematical filtration to enhance edges , and ( d ) correction for beam hardening .
	manualset3
244809	9	422246	7	NULL	NULL	0	NULL	extension	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors evaluated the effect of four types of data manipulation : ( a ) reconstruction of data with different convolution filters ( target reconstruction ) , ( b ) extension of the range of CT numbers , ( c ) mathematical filtration to enhance edges , and ( d ) correction for beam hardening .
	manualset3
244810	10	422246	7	NULL	NULL	0	NULL	 range 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors evaluated the effect of four types of data manipulation : ( a ) reconstruction of data with different convolution filters ( target reconstruction ) , ( b ) extension of the range of CT numbers , ( c ) mathematical filtration to enhance edges , and ( d ) correction for beam hardening .
	manualset3
244811	11	422246	7	NULL	NULL	0	NULL	CT numbers 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors evaluated the effect of four types of data manipulation : ( a ) reconstruction of data with different convolution filters ( target reconstruction ) , ( b ) extension of the range of CT numbers , ( c ) mathematical filtration to enhance edges , and ( d ) correction for beam hardening .
	manualset3
244812	12	422246	7	NULL	NULL	0	NULL	mathematical filtration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors evaluated the effect of four types of data manipulation : ( a ) reconstruction of data with different convolution filters ( target reconstruction ) , ( b ) extension of the range of CT numbers , ( c ) mathematical filtration to enhance edges , and ( d ) correction for beam hardening .
	manualset3
244813	13	422246	7	NULL	NULL	0	NULL	 edges 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors evaluated the effect of four types of data manipulation : ( a ) reconstruction of data with different convolution filters ( target reconstruction ) , ( b ) extension of the range of CT numbers , ( c ) mathematical filtration to enhance edges , and ( d ) correction for beam hardening .
	manualset3
244814	14	422246	7	NULL	NULL	0	NULL	correction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors evaluated the effect of four types of data manipulation : ( a ) reconstruction of data with different convolution filters ( target reconstruction ) , ( b ) extension of the range of CT numbers , ( c ) mathematical filtration to enhance edges , and ( d ) correction for beam hardening .
	manualset3
244815	15	422246	7	NULL	NULL	0	NULL	beam hardening	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The authors evaluated the effect of four types of data manipulation : ( a ) reconstruction of data with different convolution filters ( target reconstruction ) , ( b ) extension of the range of CT numbers , ( c ) mathematical filtration to enhance edges , and ( d ) correction for beam hardening .
	manualset3
244816	1	422247	7	NULL	NULL	0	NULL	protein complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	A protein complex containing Mdm10p , Mdm12p , and Mmm1p links mitochondrial membranes and DNA to the cytoskeleton-based segregation machinery .
	manualset3
244817	2	422247	7	NULL	NULL	0	NULL	Mdm10p	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A protein complex containing Mdm10p , Mdm12p , and Mmm1p links mitochondrial membranes and DNA to the cytoskeleton-based segregation machinery .
	manualset3
244818	3	422247	7	NULL	NULL	0	NULL	Mdm12p	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A protein complex containing Mdm10p , Mdm12p , and Mmm1p links mitochondrial membranes and DNA to the cytoskeleton-based segregation machinery .
	manualset3
244819	4	422247	7	NULL	NULL	0	NULL	Mmm1p	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	A protein complex containing Mdm10p , Mdm12p , and Mmm1p links mitochondrial membranes and DNA to the cytoskeleton-based segregation machinery .
	manualset3
244820	5	422247	7	NULL	NULL	0	NULL	mitochondrial membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A protein complex containing Mdm10p , Mdm12p , and Mmm1p links mitochondrial membranes and DNA to the cytoskeleton-based segregation machinery .
	manualset3
244821	6	422247	7	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A protein complex containing Mdm10p , Mdm12p , and Mmm1p links mitochondrial membranes and DNA to the cytoskeleton-based segregation machinery .
	manualset3
244822	7	422247	7	NULL	NULL	0	NULL	cytoskeleton-based segregation machinery 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	A protein complex containing Mdm10p , Mdm12p , and Mmm1p links mitochondrial membranes and DNA to the cytoskeleton-based segregation machinery .
	manualset3
244823	1	422248	7	NULL	NULL	0	NULL	extremely high titer	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An extremely high titer of platelet-associated IgG was found which was independent of the presence of carbamazepine .
	manualset3
244824	2	422248	7	NULL	NULL	0	NULL	platelet-associated IgG	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	An extremely high titer of platelet-associated IgG was found which was independent of the presence of carbamazepine .
	manualset3
244825	3	422248	7	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An extremely high titer of platelet-associated IgG was found which was independent of the presence of carbamazepine .
	manualset3
244826	4	422248	7	NULL	NULL	0	NULL	carbamazepine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An extremely high titer of platelet-associated IgG was found which was independent of the presence of carbamazepine .
	manualset3
244827	1	422249	7	NULL	NULL	0	NULL	Experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Experience with Papanicolaou stains in the study of gastric contents .
	manualset3
244828	2	422249	7	NULL	NULL	0	NULL	Papanicolaou stains	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Experience with Papanicolaou stains in the study of gastric contents .
	manualset3
244829	3	422249	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Experience with Papanicolaou stains in the study of gastric contents .
	manualset3
244830	4	422249	7	NULL	NULL	0	NULL	gastric contents	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Experience with Papanicolaou stains in the study of gastric contents .
	manualset3
244831	1	422250	7	NULL	NULL	0	NULL	Postactivation excitation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Postactivation excitation was most prominent in cells that were not spontaneously active , and decreased steadily throughout development , probably because of the steady increase in spontaneous firing rate seen during maturation .
	manualset3
244832	2	422250	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Postactivation excitation was most prominent in cells that were not spontaneously active , and decreased steadily throughout development , probably because of the steady increase in spontaneous firing rate seen during maturation .
	manualset3
244833	3	422250	7	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Postactivation excitation was most prominent in cells that were not spontaneously active , and decreased steadily throughout development , probably because of the steady increase in spontaneous firing rate seen during maturation .
	manualset3
244834	4	422250	7	NULL	NULL	0	NULL	steady increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Postactivation excitation was most prominent in cells that were not spontaneously active , and decreased steadily throughout development , probably because of the steady increase in spontaneous firing rate seen during maturation .
	manualset3
244835	5	422250	7	NULL	NULL	0	NULL	spontaneous firing rate	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Postactivation excitation was most prominent in cells that were not spontaneously active , and decreased steadily throughout development , probably because of the steady increase in spontaneous firing rate seen during maturation .
	manualset3
244836	6	422250	7	NULL	NULL	0	NULL	maturation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Postactivation excitation was most prominent in cells that were not spontaneously active , and decreased steadily throughout development , probably because of the steady increase in spontaneous firing rate seen during maturation .
	manualset3
244837	1	422251	7	NULL	NULL	0	NULL	Seven patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven patients died between 1 day and 19 months after implantation .
	manualset3
244838	2	422251	7	NULL	NULL	0	NULL	1 day	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven patients died between 1 day and 19 months after implantation .
	manualset3
244839	3	422251	7	NULL	NULL	0	NULL	19 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven patients died between 1 day and 19 months after implantation .
	manualset3
244840	4	422251	7	NULL	NULL	0	NULL	 implantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Seven patients died between 1 day and 19 months after implantation .
	manualset3
244841	1	422252	7	NULL	NULL	0	NULL	Determination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Determination of human ketone body kinetics using stable-isotope labeled tracers .
	manualset3
244842	2	422252	7	NULL	NULL	0	NULL	human ketone body kinetics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Determination of human ketone body kinetics using stable-isotope labeled tracers .
	manualset3
244843	3	422252	7	NULL	NULL	0	NULL	stable-isotope labeled tracers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Determination of human ketone body kinetics using stable-isotope labeled tracers .
	manualset3
244844	1	422253	7	NULL	NULL	0	NULL	recruitment phoenix	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The recruitment phoenix : strategies for attracting medical students into obstetrics and gynecology .
	manualset3
244845	2	422253	7	NULL	NULL	0	NULL	strategies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The recruitment phoenix : strategies for attracting medical students into obstetrics and gynecology .
	manualset3
244846	3	422253	7	NULL	NULL	0	NULL	 medical students	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The recruitment phoenix : strategies for attracting medical students into obstetrics and gynecology .
	manualset3
244847	4	422253	7	NULL	NULL	0	NULL	obstetrics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The recruitment phoenix : strategies for attracting medical students into obstetrics and gynecology .
	manualset3
244848	5	422253	7	NULL	NULL	0	NULL	gynecology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The recruitment phoenix : strategies for attracting medical students into obstetrics and gynecology .
	manualset3
244849	1	422254	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide an important link between changes in the ergosterol biosynthetic pathway and azole resistance in this opportunistic fungal species .
	manualset3
244850	2	422254	7	NULL	NULL	0	NULL	changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide an important link between changes in the ergosterol biosynthetic pathway and azole resistance in this opportunistic fungal species .
	manualset3
244851	3	422254	7	NULL	NULL	0	NULL	ergosterol biosynthetic pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide an important link between changes in the ergosterol biosynthetic pathway and azole resistance in this opportunistic fungal species .
	manualset3
244852	4	422254	7	NULL	NULL	0	NULL	azole resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide an important link between changes in the ergosterol biosynthetic pathway and azole resistance in this opportunistic fungal species .
	manualset3
244853	5	422254	7	NULL	NULL	NULL	NULL	opportunistic fungal species	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	These results provide an important link between changes in the ergosterol biosynthetic pathway and azole resistance in this opportunistic fungal species .
	manualset3
244854	6	422254	7	NULL	NULL	0	NULL	 important link 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These results provide an important link between changes in the ergosterol biosynthetic pathway and azole resistance in this opportunistic fungal species .
	manualset3
244855	2	422255	7	NULL	NULL	NULL	NULL	functional state	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This served as the reference for the functional state of other active units during the prolonged contraction .
	manualset3
244856	1	422255	7	NULL	NULL	0	NULL	reference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This served as the reference for the functional state of other active units during the prolonged contraction .
	manualset3
244857	3	422255	7	NULL	NULL	NULL	NULL	active units	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This served as the reference for the functional state of other active units during the prolonged contraction .
	manualset3
244858	4	422255	7	NULL	NULL	0	NULL	prolonged contraction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This served as the reference for the functional state of other active units during the prolonged contraction .
	manualset3
244859	1	422256	7	NULL	NULL	0	NULL	Observation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Observation of nanojet-induced modes with small propagation losses in chains of coupled spherical cavities .
	manualset3
244860	2	422256	7	NULL	NULL	0	NULL	nanojet-induced modes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Observation of nanojet-induced modes with small propagation losses in chains of coupled spherical cavities .
	manualset3
244861	3	422256	7	NULL	NULL	0	NULL	small propagation losses	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Observation of nanojet-induced modes with small propagation losses in chains of coupled spherical cavities .
	manualset3
244862	4	422256	7	NULL	NULL	0	NULL	chains 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Observation of nanojet-induced modes with small propagation losses in chains of coupled spherical cavities .
	manualset3
244863	5	422256	7	NULL	NULL	0	NULL	coupled spherical cavities	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Observation of nanojet-induced modes with small propagation losses in chains of coupled spherical cavities .
	manualset3
244864	1	422257	7	NULL	NULL	0	NULL	 range of motion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The range of motion was limited in 37 hips ( 27 % ) , and 13 hips were unstable ( 9.6 % ) .
	manualset3
244865	2	422257	7	NULL	NULL	0	NULL	37 hips	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The range of motion was limited in 37 hips ( 27 % ) , and 13 hips were unstable ( 9.6 % ) .
	manualset3
244866	3	422257	7	NULL	NULL	0	NULL	27 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The range of motion was limited in 37 hips ( 27 % ) , and 13 hips were unstable ( 9.6 % ) .
	manualset3
244867	4	422257	7	NULL	NULL	0	NULL	13 hips	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The range of motion was limited in 37 hips ( 27 % ) , and 13 hips were unstable ( 9.6 % ) .
	manualset3
244868	5	422257	7	NULL	NULL	0	NULL	9.6 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The range of motion was limited in 37 hips ( 27 % ) , and 13 hips were unstable ( 9.6 % ) .
	manualset3
244869	1	422258	7	NULL	NULL	0	NULL	Comparative studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative studies on GOD using GdmCl and NaCl demonstrated that binding of the Gdm ( + ) cation to the enzyme results in stabilization of the compact dimeric intermediate of the enzyme at low GdmCl concentrations .
	manualset3
244870	2	422258	7	NULL	NULL	0	NULL	GOD	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative studies on GOD using GdmCl and NaCl demonstrated that binding of the Gdm ( + ) cation to the enzyme results in stabilization of the compact dimeric intermediate of the enzyme at low GdmCl concentrations .
	manualset3
244871	3	422258	7	NULL	NULL	0	NULL	GdmCl 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative studies on GOD using GdmCl and NaCl demonstrated that binding of the Gdm ( + ) cation to the enzyme results in stabilization of the compact dimeric intermediate of the enzyme at low GdmCl concentrations .
	manualset3
244872	4	422258	7	NULL	NULL	0	NULL	NaCl 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative studies on GOD using GdmCl and NaCl demonstrated that binding of the Gdm ( + ) cation to the enzyme results in stabilization of the compact dimeric intermediate of the enzyme at low GdmCl concentrations .
	manualset3
244873	5	422258	7	NULL	NULL	0	NULL	binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative studies on GOD using GdmCl and NaCl demonstrated that binding of the Gdm ( + ) cation to the enzyme results in stabilization of the compact dimeric intermediate of the enzyme at low GdmCl concentrations .
	manualset3
244874	6	422258	7	NULL	NULL	0	NULL	Gdm ( + ) cation	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative studies on GOD using GdmCl and NaCl demonstrated that binding of the Gdm ( + ) cation to the enzyme results in stabilization of the compact dimeric intermediate of the enzyme at low GdmCl concentrations .
	manualset3
244875	7	422258	7	NULL	NULL	NULL	NULL	enzyme	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Comparative studies on GOD using GdmCl and NaCl demonstrated that binding of the Gdm ( + ) cation to the enzyme results in stabilization of the compact dimeric intermediate of the enzyme at low GdmCl concentrations .
	manualset3
244876	8	422258	7	NULL	NULL	0	NULL	stabilization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative studies on GOD using GdmCl and NaCl demonstrated that binding of the Gdm ( + ) cation to the enzyme results in stabilization of the compact dimeric intermediate of the enzyme at low GdmCl concentrations .
	manualset3
244877	9	422258	7	NULL	NULL	0	NULL	compact dimeric intermediate	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative studies on GOD using GdmCl and NaCl demonstrated that binding of the Gdm ( + ) cation to the enzyme results in stabilization of the compact dimeric intermediate of the enzyme at low GdmCl concentrations .
	manualset3
244878	10	422258	7	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative studies on GOD using GdmCl and NaCl demonstrated that binding of the Gdm ( + ) cation to the enzyme results in stabilization of the compact dimeric intermediate of the enzyme at low GdmCl concentrations .
	manualset3
244879	11	422258	7	NULL	NULL	0	NULL	low GdmCl concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative studies on GOD using GdmCl and NaCl demonstrated that binding of the Gdm ( + ) cation to the enzyme results in stabilization of the compact dimeric intermediate of the enzyme at low GdmCl concentrations .
	manualset3
244880	1	422259	7	NULL	NULL	0	NULL	Coma depth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Coma depth was assessed by the Glacow Coma Scale and artifact-free HR , SCL , and SCR were measured 75 times in the patient group .
	manualset3
244881	2	422259	7	NULL	NULL	0	NULL	Glacow Coma Scale	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Coma depth was assessed by the Glacow Coma Scale and artifact-free HR , SCL , and SCR were measured 75 times in the patient group .
	manualset3
244882	3	422259	7	NULL	NULL	0	NULL	artifact-free HR	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Coma depth was assessed by the Glacow Coma Scale and artifact-free HR , SCL , and SCR were measured 75 times in the patient group .
	manualset3
244883	4	422259	7	NULL	NULL	0	NULL	SCL	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Coma depth was assessed by the Glacow Coma Scale and artifact-free HR , SCL , and SCR were measured 75 times in the patient group .
	manualset3
244884	5	422259	7	NULL	NULL	0	NULL	SCR 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Coma depth was assessed by the Glacow Coma Scale and artifact-free HR , SCL , and SCR were measured 75 times in the patient group .
	manualset3
244885	6	422259	7	NULL	NULL	0	NULL	75 times	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Coma depth was assessed by the Glacow Coma Scale and artifact-free HR , SCL , and SCR were measured 75 times in the patient group .
	manualset3
244886	7	422259	7	NULL	NULL	0	NULL	patient group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Coma depth was assessed by the Glacow Coma Scale and artifact-free HR , SCL , and SCR were measured 75 times in the patient group .
	manualset3
244887	1	422260	7	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This study investigated effects of propafenone on the pharmacokinetics of caffeine .
	manualset3
244888	2	422260	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This study investigated effects of propafenone on the pharmacokinetics of caffeine .
	manualset3
244889	3	422260	7	NULL	NULL	0	NULL	propafenone 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	This study investigated effects of propafenone on the pharmacokinetics of caffeine .
	manualset3
244890	4	422260	7	NULL	NULL	0	NULL	pharmacokinetics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This study investigated effects of propafenone on the pharmacokinetics of caffeine .
	manualset3
244891	5	422260	7	NULL	NULL	0	NULL	caffeine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	This study investigated effects of propafenone on the pharmacokinetics of caffeine .
	manualset3
244892	1	422261	7	NULL	NULL	0	NULL	Administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Administration of a combination of chloroquine and the copper-lysine complex , copper ( lysine ) ( 2 ) , an inhibitor of microsomal monooxygenases , considerably decreased the parasitemia level of mice infected with a chloroquine-resistant strain of Plasmodium berghei .
	manualset3
244893	2	422261	7	NULL	NULL	0	NULL	combination	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Administration of a combination of chloroquine and the copper-lysine complex , copper ( lysine ) ( 2 ) , an inhibitor of microsomal monooxygenases , considerably decreased the parasitemia level of mice infected with a chloroquine-resistant strain of Plasmodium berghei .
	manualset3
244894	3	422261	7	NULL	NULL	0	NULL	chloroquine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Administration of a combination of chloroquine and the copper-lysine complex , copper ( lysine ) ( 2 ) , an inhibitor of microsomal monooxygenases , considerably decreased the parasitemia level of mice infected with a chloroquine-resistant strain of Plasmodium berghei .
	manualset3
244895	4	422261	7	NULL	NULL	0	NULL	copper-lysine complex	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Administration of a combination of chloroquine and the copper-lysine complex , copper ( lysine ) ( 2 ) , an inhibitor of microsomal monooxygenases , considerably decreased the parasitemia level of mice infected with a chloroquine-resistant strain of Plasmodium berghei .
	manualset3
244896	5	422261	7	NULL	NULL	0	NULL	copper ( lysine ) ( 2 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Administration of a combination of chloroquine and the copper-lysine complex , copper ( lysine ) ( 2 ) , an inhibitor of microsomal monooxygenases , considerably decreased the parasitemia level of mice infected with a chloroquine-resistant strain of Plasmodium berghei .
	manualset3
244897	6	422261	7	NULL	NULL	0	NULL	 inhibitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Administration of a combination of chloroquine and the copper-lysine complex , copper ( lysine ) ( 2 ) , an inhibitor of microsomal monooxygenases , considerably decreased the parasitemia level of mice infected with a chloroquine-resistant strain of Plasmodium berghei .
	manualset3
244898	7	422261	7	NULL	NULL	0	NULL	microsomal monooxygenases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Administration of a combination of chloroquine and the copper-lysine complex , copper ( lysine ) ( 2 ) , an inhibitor of microsomal monooxygenases , considerably decreased the parasitemia level of mice infected with a chloroquine-resistant strain of Plasmodium berghei .
	manualset3
244899	8	422261	7	NULL	NULL	NULL	NULL	parasitemia level	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Administration of a combination of chloroquine and the copper-lysine complex , copper ( lysine ) ( 2 ) , an inhibitor of microsomal monooxygenases , considerably decreased the parasitemia level of mice infected with a chloroquine-resistant strain of Plasmodium berghei .
	manualset3
244900	9	422261	7	NULL	NULL	0	NULL	 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Administration of a combination of chloroquine and the copper-lysine complex , copper ( lysine ) ( 2 ) , an inhibitor of microsomal monooxygenases , considerably decreased the parasitemia level of mice infected with a chloroquine-resistant strain of Plasmodium berghei .
	manualset3
244901	10	422261	7	NULL	NULL	0	NULL	chloroquine-resistant strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Administration of a combination of chloroquine and the copper-lysine complex , copper ( lysine ) ( 2 ) , an inhibitor of microsomal monooxygenases , considerably decreased the parasitemia level of mice infected with a chloroquine-resistant strain of Plasmodium berghei .
	manualset3
244902	11	422261	7	NULL	NULL	0	NULL	Plasmodium berghei	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Administration of a combination of chloroquine and the copper-lysine complex , copper ( lysine ) ( 2 ) , an inhibitor of microsomal monooxygenases , considerably decreased the parasitemia level of mice infected with a chloroquine-resistant strain of Plasmodium berghei .
	manualset3
244903	1	422262	7	NULL	NULL	0	NULL	 small amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When a small amount ( 2 micrograms ) of SEB was employed , it did not stimulate T cell expansion in AKR/J mice .
	manualset3
244904	2	422262	7	NULL	NULL	0	NULL	2 micrograms	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	When a small amount ( 2 micrograms ) of SEB was employed , it did not stimulate T cell expansion in AKR/J mice .
	manualset3
244905	3	422262	7	NULL	NULL	0	NULL	SEB	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When a small amount ( 2 micrograms ) of SEB was employed , it did not stimulate T cell expansion in AKR/J mice .
	manualset3
244906	4	422262	7	NULL	NULL	0	NULL	T cell expansion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	When a small amount ( 2 micrograms ) of SEB was employed , it did not stimulate T cell expansion in AKR/J mice .
	manualset3
244907	5	422262	7	NULL	NULL	0	NULL	AKR/J mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	When a small amount ( 2 micrograms ) of SEB was employed , it did not stimulate T cell expansion in AKR/J mice .
	manualset3
244908	1	422263	7	NULL	NULL	0	NULL	identical effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An identical effect was seen after exposure to 20 + 200 micrograms/L Ag + Cu in the long-term action ( 24 h of incubation ) .
	manualset3
244909	2	422263	7	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An identical effect was seen after exposure to 20 + 200 micrograms/L Ag + Cu in the long-term action ( 24 h of incubation ) .
	manualset3
244910	3	422263	7	NULL	NULL	0	NULL	20 + 200 micrograms/L 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An identical effect was seen after exposure to 20 + 200 micrograms/L Ag + Cu in the long-term action ( 24 h of incubation ) .
	manualset3
244911	4	422263	7	NULL	NULL	0	NULL	Ag + Cu	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	An identical effect was seen after exposure to 20 + 200 micrograms/L Ag + Cu in the long-term action ( 24 h of incubation ) .
	manualset3
244912	5	422263	7	NULL	NULL	0	NULL	long-term action	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An identical effect was seen after exposure to 20 + 200 micrograms/L Ag + Cu in the long-term action ( 24 h of incubation ) .
	manualset3
244913	6	422263	7	NULL	NULL	0	NULL	24 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	An identical effect was seen after exposure to 20 + 200 micrograms/L Ag + Cu in the long-term action ( 24 h of incubation ) .
	manualset3
244914	7	422263	7	NULL	NULL	0	NULL	incubation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An identical effect was seen after exposure to 20 + 200 micrograms/L Ag + Cu in the long-term action ( 24 h of incubation ) .
	manualset3
244915	1	422264	7	NULL	NULL	0	NULL	voluntary anorexia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This voluntary anorexia was accompanied by substantial weight loss , and the anorexia was rapidly reversed by removal of the running wheels .
	manualset3
244916	2	422264	7	NULL	NULL	0	NULL	weight loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This voluntary anorexia was accompanied by substantial weight loss , and the anorexia was rapidly reversed by removal of the running wheels .
	manualset3
244917	3	422264	7	NULL	NULL	0	NULL	anorexia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This voluntary anorexia was accompanied by substantial weight loss , and the anorexia was rapidly reversed by removal of the running wheels .
	manualset3
244918	4	422264	7	NULL	NULL	0	NULL	 removal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This voluntary anorexia was accompanied by substantial weight loss , and the anorexia was rapidly reversed by removal of the running wheels .
	manualset3
244919	5	422264	7	NULL	NULL	0	NULL	running wheels	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	This voluntary anorexia was accompanied by substantial weight loss , and the anorexia was rapidly reversed by removal of the running wheels .
	manualset3
244920	1	422265	7	NULL	NULL	0	NULL	hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , the hepatocytes were exposed directly to circulating blood cells and had degenerative changes with accumulation of red blood cells in the cytoplasm .
	manualset3
244921	2	422265	7	NULL	NULL	0	NULL	circulating blood cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , the hepatocytes were exposed directly to circulating blood cells and had degenerative changes with accumulation of red blood cells in the cytoplasm .
	manualset3
244922	3	422265	7	NULL	NULL	0	NULL	degenerative changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , the hepatocytes were exposed directly to circulating blood cells and had degenerative changes with accumulation of red blood cells in the cytoplasm .
	manualset3
244923	4	422265	7	NULL	NULL	0	NULL	accumulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , the hepatocytes were exposed directly to circulating blood cells and had degenerative changes with accumulation of red blood cells in the cytoplasm .
	manualset3
244924	5	422265	7	NULL	NULL	0	NULL	red blood cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , the hepatocytes were exposed directly to circulating blood cells and had degenerative changes with accumulation of red blood cells in the cytoplasm .
	manualset3
244925	6	422265	7	NULL	NULL	0	NULL	cytoplasm	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Subsequently , the hepatocytes were exposed directly to circulating blood cells and had degenerative changes with accumulation of red blood cells in the cytoplasm .
	manualset3
244926	1	422266	7	NULL	NULL	0	NULL	low expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the low expression of islet-1 mRNA made it necessary to develop a two-step amplification procedure in order to provide a reliable semiquantitative analysis .
	manualset3
244927	2	422266	7	NULL	NULL	0	NULL	islet-1 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the low expression of islet-1 mRNA made it necessary to develop a two-step amplification procedure in order to provide a reliable semiquantitative analysis .
	manualset3
244928	3	422266	7	NULL	NULL	0	NULL	two-step amplification procedure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the low expression of islet-1 mRNA made it necessary to develop a two-step amplification procedure in order to provide a reliable semiquantitative analysis .
	manualset3
244929	4	422266	7	NULL	NULL	0	NULL	semiquantitative analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In contrast , the low expression of islet-1 mRNA made it necessary to develop a two-step amplification procedure in order to provide a reliable semiquantitative analysis .
	manualset3
244930	1	422267	7	NULL	NULL	0	NULL	 paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	This paper introduces a new method for the interpolation that has to be performed when motion estimation and compensation are applied to interlaced sequences with subpel accuracy .
	manualset3
244931	2	422267	7	NULL	NULL	0	NULL	new method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This paper introduces a new method for the interpolation that has to be performed when motion estimation and compensation are applied to interlaced sequences with subpel accuracy .
	manualset3
244932	3	422267	7	NULL	NULL	0	NULL	interpolation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This paper introduces a new method for the interpolation that has to be performed when motion estimation and compensation are applied to interlaced sequences with subpel accuracy .
	manualset3
244933	4	422267	7	NULL	NULL	0	NULL	motion estimation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This paper introduces a new method for the interpolation that has to be performed when motion estimation and compensation are applied to interlaced sequences with subpel accuracy .
	manualset3
244934	5	422267	7	NULL	NULL	0	NULL	compensation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This paper introduces a new method for the interpolation that has to be performed when motion estimation and compensation are applied to interlaced sequences with subpel accuracy .
	manualset3
244935	6	422267	7	NULL	NULL	0	NULL	interlaced sequences	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	This paper introduces a new method for the interpolation that has to be performed when motion estimation and compensation are applied to interlaced sequences with subpel accuracy .
	manualset3
244936	7	422267	7	NULL	NULL	0	NULL	subpel accuracy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This paper introduces a new method for the interpolation that has to be performed when motion estimation and compensation are applied to interlaced sequences with subpel accuracy .
	manualset3
244937	1	422268	7	NULL	NULL	0	NULL	standing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	During standing , all participants wore a harness and were suspended by an overhead , pneumatic body weight support ( BWS ) system over a treadmill .
	manualset3
244938	2	422268	7	NULL	NULL	0	NULL	participants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	During standing , all participants wore a harness and were suspended by an overhead , pneumatic body weight support ( BWS ) system over a treadmill .
	manualset3
244939	3	422268	7	NULL	NULL	NULL	NULL	pneumatic body weight support ( BWS ) system	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During standing , all participants wore a harness and were suspended by an overhead , pneumatic body weight support ( BWS ) system over a treadmill .
	manualset3
244940	4	422268	7	NULL	NULL	0	NULL	treadmill	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	During standing , all participants wore a harness and were suspended by an overhead , pneumatic body weight support ( BWS ) system over a treadmill .
	manualset3
244941	1	422269	7	NULL	NULL	0	NULL	Global gene expression analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Global gene expression analysis was performed on total vertebrae from wild-type ( WT ) and TRalpha1 - / - beta - / - mice using DNA microarray and the results were verified by real-time PCR .
	manualset3
244942	2	422269	7	NULL	NULL	0	NULL	total vertebrae	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Global gene expression analysis was performed on total vertebrae from wild-type ( WT ) and TRalpha1 - / - beta - / - mice using DNA microarray and the results were verified by real-time PCR .
	manualset3
244943	3	422269	7	NULL	NULL	0	NULL	wild-type ( WT ) mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Global gene expression analysis was performed on total vertebrae from wild-type ( WT ) and TRalpha1 - / - beta - / - mice using DNA microarray and the results were verified by real-time PCR .
	manualset3
244944	4	422269	7	NULL	NULL	0	NULL	TRalpha1 - / - beta - / - mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Global gene expression analysis was performed on total vertebrae from wild-type ( WT ) and TRalpha1 - / - beta - / - mice using DNA microarray and the results were verified by real-time PCR .
	manualset3
244945	5	422269	7	NULL	NULL	0	NULL	DNA microarray	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Global gene expression analysis was performed on total vertebrae from wild-type ( WT ) and TRalpha1 - / - beta - / - mice using DNA microarray and the results were verified by real-time PCR .
	manualset3
244946	6	422269	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Global gene expression analysis was performed on total vertebrae from wild-type ( WT ) and TRalpha1 - / - beta - / - mice using DNA microarray and the results were verified by real-time PCR .
	manualset3
244947	7	422269	7	NULL	NULL	0	NULL	real-time PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Global gene expression analysis was performed on total vertebrae from wild-type ( WT ) and TRalpha1 - / - beta - / - mice using DNA microarray and the results were verified by real-time PCR .
	manualset3
244948	1	422270	7	NULL	NULL	0	NULL	 factors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Influencing factors such as co-substrate , temperature and pH were optimized through batch experiments .
	manualset3
244949	2	422270	7	NULL	NULL	0	NULL	co-substrate 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Influencing factors such as co-substrate , temperature and pH were optimized through batch experiments .
	manualset3
244950	3	422270	7	NULL	NULL	0	NULL	temperature	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Influencing factors such as co-substrate , temperature and pH were optimized through batch experiments .
	manualset3
244951	4	422270	7	NULL	NULL	0	NULL	pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Influencing factors such as co-substrate , temperature and pH were optimized through batch experiments .
	manualset3
244952	5	422270	7	NULL	NULL	NULL	NULL	batch experiments	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Influencing factors such as co-substrate , temperature and pH were optimized through batch experiments .
	manualset3
244953	1	422271	7	NULL	NULL	0	NULL	Nuclei 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclei prepared from young adult and senescent Caenorhabditis elegans ( Nematoda ) were subjected to digestion by micrococcal nuclease and DNaseI .
	manualset3
244954	2	422271	7	NULL	NULL	0	NULL	 young adult	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclei prepared from young adult and senescent Caenorhabditis elegans ( Nematoda ) were subjected to digestion by micrococcal nuclease and DNaseI .
	manualset3
244955	3	422271	7	NULL	NULL	0	NULL	Caenorhabditis elegans ( Nematoda )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclei prepared from young adult and senescent Caenorhabditis elegans ( Nematoda ) were subjected to digestion by micrococcal nuclease and DNaseI .
	manualset3
244956	4	422271	7	NULL	NULL	0	NULL	digestion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclei prepared from young adult and senescent Caenorhabditis elegans ( Nematoda ) were subjected to digestion by micrococcal nuclease and DNaseI .
	manualset3
244957	5	422271	7	NULL	NULL	0	NULL	micrococcal nuclease 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclei prepared from young adult and senescent Caenorhabditis elegans ( Nematoda ) were subjected to digestion by micrococcal nuclease and DNaseI .
	manualset3
244958	6	422271	7	NULL	NULL	0	NULL	DNaseI	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nuclei prepared from young adult and senescent Caenorhabditis elegans ( Nematoda ) were subjected to digestion by micrococcal nuclease and DNaseI .
	manualset3
244959	1	422272	7	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This study aimed to explore the relationship between TNF - and ovariectomy induced hyperalgesia .
	manualset3
244960	2	422272	7	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	This study aimed to explore the relationship between TNF - and ovariectomy induced hyperalgesia .
	manualset3
244961	3	422272	7	NULL	NULL	0	NULL	TNF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This study aimed to explore the relationship between TNF - and ovariectomy induced hyperalgesia .
	manualset3
244962	4	422272	7	NULL	NULL	0	NULL	ovariectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This study aimed to explore the relationship between TNF - and ovariectomy induced hyperalgesia .
	manualset3
244963	5	422272	7	NULL	NULL	0	NULL	hyperalgesia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	This study aimed to explore the relationship between TNF - and ovariectomy induced hyperalgesia .
	manualset3
244964	1	422273	7	NULL	NULL	0	NULL	 mol wt	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The mol wt of the glycoprotein ( s ) carrying the PLA1 antigen was examined on platelets , megakaryocytes and endothelial cells by immunoblotting with a human polyclonal anti-PLA1 antibody ( BE ) , as well as on four different monoclonal antibodies ( MoAbs ; DEK-1 , DEK-2C , DEK-10 , and DEK-16 ) raised against GPIIIa , the 100 , 000-mol wt platelet glycoprotein known to carry the PLA1 antigen .
	manualset3
244965	2	422273	7	NULL	NULL	0	NULL	glycoprotein ( s )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mol wt of the glycoprotein ( s ) carrying the PLA1 antigen was examined on platelets , megakaryocytes and endothelial cells by immunoblotting with a human polyclonal anti-PLA1 antibody ( BE ) , as well as on four different monoclonal antibodies ( MoAbs ; DEK-1 , DEK-2C , DEK-10 , and DEK-16 ) raised against GPIIIa , the 100 , 000-mol wt platelet glycoprotein known to carry the PLA1 antigen .
	manualset3
244966	3	422273	7	NULL	NULL	0	NULL	PLA1 antigen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mol wt of the glycoprotein ( s ) carrying the PLA1 antigen was examined on platelets , megakaryocytes and endothelial cells by immunoblotting with a human polyclonal anti-PLA1 antibody ( BE ) , as well as on four different monoclonal antibodies ( MoAbs ; DEK-1 , DEK-2C , DEK-10 , and DEK-16 ) raised against GPIIIa , the 100 , 000-mol wt platelet glycoprotein known to carry the PLA1 antigen .
	manualset3
244967	4	422273	7	NULL	NULL	0	NULL	platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The mol wt of the glycoprotein ( s ) carrying the PLA1 antigen was examined on platelets , megakaryocytes and endothelial cells by immunoblotting with a human polyclonal anti-PLA1 antibody ( BE ) , as well as on four different monoclonal antibodies ( MoAbs ; DEK-1 , DEK-2C , DEK-10 , and DEK-16 ) raised against GPIIIa , the 100 , 000-mol wt platelet glycoprotein known to carry the PLA1 antigen .
	manualset3
244968	5	422273	7	NULL	NULL	0	NULL	megakaryocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The mol wt of the glycoprotein ( s ) carrying the PLA1 antigen was examined on platelets , megakaryocytes and endothelial cells by immunoblotting with a human polyclonal anti-PLA1 antibody ( BE ) , as well as on four different monoclonal antibodies ( MoAbs ; DEK-1 , DEK-2C , DEK-10 , and DEK-16 ) raised against GPIIIa , the 100 , 000-mol wt platelet glycoprotein known to carry the PLA1 antigen .
	manualset3
244969	6	422273	7	NULL	NULL	0	NULL	endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The mol wt of the glycoprotein ( s ) carrying the PLA1 antigen was examined on platelets , megakaryocytes and endothelial cells by immunoblotting with a human polyclonal anti-PLA1 antibody ( BE ) , as well as on four different monoclonal antibodies ( MoAbs ; DEK-1 , DEK-2C , DEK-10 , and DEK-16 ) raised against GPIIIa , the 100 , 000-mol wt platelet glycoprotein known to carry the PLA1 antigen .
	manualset3
244970	7	422273	7	NULL	NULL	0	NULL	immunoblotting	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The mol wt of the glycoprotein ( s ) carrying the PLA1 antigen was examined on platelets , megakaryocytes and endothelial cells by immunoblotting with a human polyclonal anti-PLA1 antibody ( BE ) , as well as on four different monoclonal antibodies ( MoAbs ; DEK-1 , DEK-2C , DEK-10 , and DEK-16 ) raised against GPIIIa , the 100 , 000-mol wt platelet glycoprotein known to carry the PLA1 antigen .
	manualset3
244971	8	422273	7	NULL	NULL	0	NULL	human polyclonal anti-PLA1 antibody ( BE )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mol wt of the glycoprotein ( s ) carrying the PLA1 antigen was examined on platelets , megakaryocytes and endothelial cells by immunoblotting with a human polyclonal anti-PLA1 antibody ( BE ) , as well as on four different monoclonal antibodies ( MoAbs ; DEK-1 , DEK-2C , DEK-10 , and DEK-16 ) raised against GPIIIa , the 100 , 000-mol wt platelet glycoprotein known to carry the PLA1 antigen .
	manualset3
244972	9	422273	7	NULL	NULL	0	NULL	four different monoclonal antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The mol wt of the glycoprotein ( s ) carrying the PLA1 antigen was examined on platelets , megakaryocytes and endothelial cells by immunoblotting with a human polyclonal anti-PLA1 antibody ( BE ) , as well as on four different monoclonal antibodies ( MoAbs ; DEK-1 , DEK-2C , DEK-10 , and DEK-16 ) raised against GPIIIa , the 100 , 000-mol wt platelet glycoprotein known to carry the PLA1 antigen .
	manualset3
244973	10	422273	7	NULL	NULL	0	NULL	MoAbs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The mol wt of the glycoprotein ( s ) carrying the PLA1 antigen was examined on platelets , megakaryocytes and endothelial cells by immunoblotting with a human polyclonal anti-PLA1 antibody ( BE ) , as well as on four different monoclonal antibodies ( MoAbs ; DEK-1 , DEK-2C , DEK-10 , and DEK-16 ) raised against GPIIIa , the 100 , 000-mol wt platelet glycoprotein known to carry the PLA1 antigen .
	manualset3
244974	11	422273	7	NULL	NULL	0	NULL	DEK-1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mol wt of the glycoprotein ( s ) carrying the PLA1 antigen was examined on platelets , megakaryocytes and endothelial cells by immunoblotting with a human polyclonal anti-PLA1 antibody ( BE ) , as well as on four different monoclonal antibodies ( MoAbs ; DEK-1 , DEK-2C , DEK-10 , and DEK-16 ) raised against GPIIIa , the 100 , 000-mol wt platelet glycoprotein known to carry the PLA1 antigen .
	manualset3
244975	12	422273	7	NULL	NULL	0	NULL	DEK-2C	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mol wt of the glycoprotein ( s ) carrying the PLA1 antigen was examined on platelets , megakaryocytes and endothelial cells by immunoblotting with a human polyclonal anti-PLA1 antibody ( BE ) , as well as on four different monoclonal antibodies ( MoAbs ; DEK-1 , DEK-2C , DEK-10 , and DEK-16 ) raised against GPIIIa , the 100 , 000-mol wt platelet glycoprotein known to carry the PLA1 antigen .
	manualset3
244976	13	422273	7	NULL	NULL	0	NULL	DEK-10	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mol wt of the glycoprotein ( s ) carrying the PLA1 antigen was examined on platelets , megakaryocytes and endothelial cells by immunoblotting with a human polyclonal anti-PLA1 antibody ( BE ) , as well as on four different monoclonal antibodies ( MoAbs ; DEK-1 , DEK-2C , DEK-10 , and DEK-16 ) raised against GPIIIa , the 100 , 000-mol wt platelet glycoprotein known to carry the PLA1 antigen .
	manualset3
244977	14	422273	7	NULL	NULL	0	NULL	DEK-16	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mol wt of the glycoprotein ( s ) carrying the PLA1 antigen was examined on platelets , megakaryocytes and endothelial cells by immunoblotting with a human polyclonal anti-PLA1 antibody ( BE ) , as well as on four different monoclonal antibodies ( MoAbs ; DEK-1 , DEK-2C , DEK-10 , and DEK-16 ) raised against GPIIIa , the 100 , 000-mol wt platelet glycoprotein known to carry the PLA1 antigen .
	manualset3
244978	15	422273	7	NULL	NULL	0	NULL	GPIIIa	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mol wt of the glycoprotein ( s ) carrying the PLA1 antigen was examined on platelets , megakaryocytes and endothelial cells by immunoblotting with a human polyclonal anti-PLA1 antibody ( BE ) , as well as on four different monoclonal antibodies ( MoAbs ; DEK-1 , DEK-2C , DEK-10 , and DEK-16 ) raised against GPIIIa , the 100 , 000-mol wt platelet glycoprotein known to carry the PLA1 antigen .
	manualset3
244979	16	422273	7	NULL	NULL	0	NULL	100 , 000-mol wt	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The mol wt of the glycoprotein ( s ) carrying the PLA1 antigen was examined on platelets , megakaryocytes and endothelial cells by immunoblotting with a human polyclonal anti-PLA1 antibody ( BE ) , as well as on four different monoclonal antibodies ( MoAbs ; DEK-1 , DEK-2C , DEK-10 , and DEK-16 ) raised against GPIIIa , the 100 , 000-mol wt platelet glycoprotein known to carry the PLA1 antigen .
	manualset3
244980	17	422273	7	NULL	NULL	0	NULL	platelet glycoprotein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mol wt of the glycoprotein ( s ) carrying the PLA1 antigen was examined on platelets , megakaryocytes and endothelial cells by immunoblotting with a human polyclonal anti-PLA1 antibody ( BE ) , as well as on four different monoclonal antibodies ( MoAbs ; DEK-1 , DEK-2C , DEK-10 , and DEK-16 ) raised against GPIIIa , the 100 , 000-mol wt platelet glycoprotein known to carry the PLA1 antigen .
	manualset3
244981	18	422273	7	NULL	NULL	0	NULL	PLA1 antigen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The mol wt of the glycoprotein ( s ) carrying the PLA1 antigen was examined on platelets , megakaryocytes and endothelial cells by immunoblotting with a human polyclonal anti-PLA1 antibody ( BE ) , as well as on four different monoclonal antibodies ( MoAbs ; DEK-1 , DEK-2C , DEK-10 , and DEK-16 ) raised against GPIIIa , the 100 , 000-mol wt platelet glycoprotein known to carry the PLA1 antigen .
	manualset3
244982	1	422274	7	NULL	NULL	0	NULL	Peritoneal lavage 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Peritoneal lavage was started earlier in survivors and was effective in decreasing pain and amylase levels , but not in correcting hypoxemia .
	manualset3
244983	2	422274	7	NULL	NULL	0	NULL	 survivors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Peritoneal lavage was started earlier in survivors and was effective in decreasing pain and amylase levels , but not in correcting hypoxemia .
	manualset3
244984	3	422274	7	NULL	NULL	0	NULL	pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Peritoneal lavage was started earlier in survivors and was effective in decreasing pain and amylase levels , but not in correcting hypoxemia .
	manualset3
244985	4	422274	7	NULL	NULL	0	NULL	amylase levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Peritoneal lavage was started earlier in survivors and was effective in decreasing pain and amylase levels , but not in correcting hypoxemia .
	manualset3
244986	5	422274	7	NULL	NULL	0	NULL	hypoxemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Peritoneal lavage was started earlier in survivors and was effective in decreasing pain and amylase levels , but not in correcting hypoxemia .
	manualset3
244987	1	422275	7	NULL	NULL	0	NULL	Development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Development of a Chinese version of the Oswestry Disability Index version 2.1 .
	manualset3
244988	2	422275	7	NULL	NULL	NULL	NULL	Chinese version	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of a Chinese version of the Oswestry Disability Index version 2.1 .
	manualset3
244989	3	422275	7	NULL	NULL	NULL	NULL	Oswestry Disability Index version 2.1	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of a Chinese version of the Oswestry Disability Index version 2.1 .
	manualset3
244990	1	422276	7	NULL	NULL	0	NULL	Enamel-dentinal adhesives	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Enamel-dentinal adhesives in amalgam restorations .
	manualset3
244991	2	422276	7	NULL	NULL	0	NULL	amalgam restorations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Enamel-dentinal adhesives in amalgam restorations .
	manualset3
244992	1	422277	7	NULL	NULL	NULL	NULL	Capsaicin treatment	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Capsaicin treatment of neonatal mice , which causes a loss of unmyelinated sensory neurons , some of which contain substance P , reduced the mortality rate of HSV-infected mice .
	manualset3
244993	2	422277	7	NULL	NULL	0	NULL	neonatal mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Capsaicin treatment of neonatal mice , which causes a loss of unmyelinated sensory neurons , some of which contain substance P , reduced the mortality rate of HSV-infected mice .
	manualset3
244994	3	422277	7	NULL	NULL	0	NULL	unmyelinated sensory neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Capsaicin treatment of neonatal mice , which causes a loss of unmyelinated sensory neurons , some of which contain substance P , reduced the mortality rate of HSV-infected mice .
	manualset3
244995	4	422277	7	NULL	NULL	0	NULL	substance P	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Capsaicin treatment of neonatal mice , which causes a loss of unmyelinated sensory neurons , some of which contain substance P , reduced the mortality rate of HSV-infected mice .
	manualset3
244996	5	422277	7	NULL	NULL	0	NULL	mortality rate	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Capsaicin treatment of neonatal mice , which causes a loss of unmyelinated sensory neurons , some of which contain substance P , reduced the mortality rate of HSV-infected mice .
	manualset3
244997	6	422277	7	NULL	NULL	0	NULL	HSV-infected mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Capsaicin treatment of neonatal mice , which causes a loss of unmyelinated sensory neurons , some of which contain substance P , reduced the mortality rate of HSV-infected mice .
	manualset3
247343	7	422277	7	NULL	NULL	0	NULL	loss	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Capsaicin treatment of neonatal mice , which causes a loss of unmyelinated sensory neurons , some of which contain substance P , reduced the mortality rate of HSV-infected mice .
	manualset3
244998	1	422278	7	NULL	NULL	0	NULL	o-phthalaldehyde	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Using o-phthalaldehyde to block the Lys residue at the fourth amino acid pair from the N-terminus which leaves the Pro residue free for subsequent Edman degradation , we have deduced the N-terminal sequence of each of the two subunits for form I clusterin .
	manualset3
244999	2	422278	7	NULL	NULL	0	NULL	Lys residue	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using o-phthalaldehyde to block the Lys residue at the fourth amino acid pair from the N-terminus which leaves the Pro residue free for subsequent Edman degradation , we have deduced the N-terminal sequence of each of the two subunits for form I clusterin .
	manualset3
245000	3	422278	7	NULL	NULL	0	NULL	fourth amino acid pair 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using o-phthalaldehyde to block the Lys residue at the fourth amino acid pair from the N-terminus which leaves the Pro residue free for subsequent Edman degradation , we have deduced the N-terminal sequence of each of the two subunits for form I clusterin .
	manualset3
245001	4	422278	7	NULL	NULL	0	NULL	N-terminus	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using o-phthalaldehyde to block the Lys residue at the fourth amino acid pair from the N-terminus which leaves the Pro residue free for subsequent Edman degradation , we have deduced the N-terminal sequence of each of the two subunits for form I clusterin .
	manualset3
245002	5	422278	7	NULL	NULL	0	NULL	Pro residue	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Using o-phthalaldehyde to block the Lys residue at the fourth amino acid pair from the N-terminus which leaves the Pro residue free for subsequent Edman degradation , we have deduced the N-terminal sequence of each of the two subunits for form I clusterin .
	manualset3
245003	6	422278	7	NULL	NULL	0	NULL	Edman degradation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Using o-phthalaldehyde to block the Lys residue at the fourth amino acid pair from the N-terminus which leaves the Pro residue free for subsequent Edman degradation , we have deduced the N-terminal sequence of each of the two subunits for form I clusterin .
	manualset3
245004	7	422278	7	NULL	NULL	0	NULL	N-terminal sequence	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using o-phthalaldehyde to block the Lys residue at the fourth amino acid pair from the N-terminus which leaves the Pro residue free for subsequent Edman degradation , we have deduced the N-terminal sequence of each of the two subunits for form I clusterin .
	manualset3
245005	8	422278	7	NULL	NULL	0	NULL	 two subunits	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using o-phthalaldehyde to block the Lys residue at the fourth amino acid pair from the N-terminus which leaves the Pro residue free for subsequent Edman degradation , we have deduced the N-terminal sequence of each of the two subunits for form I clusterin .
	manualset3
245006	9	422278	7	NULL	NULL	0	NULL	 I clusterin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Using o-phthalaldehyde to block the Lys residue at the fourth amino acid pair from the N-terminus which leaves the Pro residue free for subsequent Edman degradation , we have deduced the N-terminal sequence of each of the two subunits for form I clusterin .
	manualset3
245007	1	422279	7	NULL	NULL	0	NULL	theoretical model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A theoretical model of magneto-acoustic current imaging is derived , based on fundamental equations of continuum mechanics and electromagnetism .
	manualset3
245008	2	422279	7	NULL	NULL	0	NULL	magneto-acoustic current imaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	A theoretical model of magneto-acoustic current imaging is derived , based on fundamental equations of continuum mechanics and electromagnetism .
	manualset3
245009	3	422279	7	NULL	NULL	0	NULL	fundamental equations	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A theoretical model of magneto-acoustic current imaging is derived , based on fundamental equations of continuum mechanics and electromagnetism .
	manualset3
245010	4	422279	7	NULL	NULL	0	NULL	continuum mechanics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	A theoretical model of magneto-acoustic current imaging is derived , based on fundamental equations of continuum mechanics and electromagnetism .
	manualset3
245011	5	422279	7	NULL	NULL	0	NULL	 electromagnetism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	A theoretical model of magneto-acoustic current imaging is derived , based on fundamental equations of continuum mechanics and electromagnetism .
	manualset3
245012	1	422280	7	NULL	NULL	0	NULL	Two-hybridization events	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-hybridization events have been postulated in the whole of the T. cruzi pedigree , the first of which yielded the four predominant nuclear genotypes .
	manualset3
245013	2	422280	7	NULL	NULL	0	NULL	T. cruzi pedigree	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-hybridization events have been postulated in the whole of the T. cruzi pedigree , the first of which yielded the four predominant nuclear genotypes .
	manualset3
245014	3	422280	7	NULL	NULL	0	NULL	first	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-hybridization events have been postulated in the whole of the T. cruzi pedigree , the first of which yielded the four predominant nuclear genotypes .
	manualset3
245015	4	422280	7	NULL	NULL	0	NULL	four predominant nuclear genotypes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Two-hybridization events have been postulated in the whole of the T. cruzi pedigree , the first of which yielded the four predominant nuclear genotypes .
	manualset3
245016	1	422281	7	NULL	NULL	0	NULL	Lower disease activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lower disease activity and disability in Swedish patients with rheumatoid arthritis in 1995 compared with 1978 .
	manualset3
245017	2	422281	7	NULL	NULL	0	NULL	disability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Lower disease activity and disability in Swedish patients with rheumatoid arthritis in 1995 compared with 1978 .
	manualset3
245018	3	422281	7	NULL	NULL	0	NULL	Swedish patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Lower disease activity and disability in Swedish patients with rheumatoid arthritis in 1995 compared with 1978 .
	manualset3
245019	4	422281	7	NULL	NULL	0	NULL	 rheumatoid arthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Lower disease activity and disability in Swedish patients with rheumatoid arthritis in 1995 compared with 1978 .
	manualset3
245020	5	422281	7	NULL	NULL	0	NULL	1995	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Lower disease activity and disability in Swedish patients with rheumatoid arthritis in 1995 compared with 1978 .
	manualset3
245021	6	422281	7	NULL	NULL	0	NULL	1978	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Lower disease activity and disability in Swedish patients with rheumatoid arthritis in 1995 compared with 1978 .
	manualset3
245022	1	422282	7	NULL	NULL	0	NULL	Changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Changes of the activity and content of sucrase-isomaltase complex in the intestinal mucosa during the development of streptozotocin-induced diabetes in rats .
	manualset3
245023	2	422282	7	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Changes of the activity and content of sucrase-isomaltase complex in the intestinal mucosa during the development of streptozotocin-induced diabetes in rats .
	manualset3
245024	3	422282	7	NULL	NULL	0	NULL	content	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Changes of the activity and content of sucrase-isomaltase complex in the intestinal mucosa during the development of streptozotocin-induced diabetes in rats .
	manualset3
245025	4	422282	7	NULL	NULL	0	NULL	sucrase-isomaltase complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Changes of the activity and content of sucrase-isomaltase complex in the intestinal mucosa during the development of streptozotocin-induced diabetes in rats .
	manualset3
245026	5	422282	7	NULL	NULL	0	NULL	intestinal mucosa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Changes of the activity and content of sucrase-isomaltase complex in the intestinal mucosa during the development of streptozotocin-induced diabetes in rats .
	manualset3
245027	6	422282	7	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Changes of the activity and content of sucrase-isomaltase complex in the intestinal mucosa during the development of streptozotocin-induced diabetes in rats .
	manualset3
245028	7	422282	7	NULL	NULL	0	NULL	streptozotocin-induced diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Changes of the activity and content of sucrase-isomaltase complex in the intestinal mucosa during the development of streptozotocin-induced diabetes in rats .
	manualset3
245029	8	422282	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Changes of the activity and content of sucrase-isomaltase complex in the intestinal mucosa during the development of streptozotocin-induced diabetes in rats .
	manualset3
245030	1	422283	7	NULL	NULL	NULL	NULL	 imbalance	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An imbalance of ascending dopaminergic tracts may drive rapid fluctuations in level of arousal and in the associated mood , drive and motivation .
	manualset3
245031	2	422283	7	NULL	NULL	0	NULL	ascending dopaminergic tracts	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An imbalance of ascending dopaminergic tracts may drive rapid fluctuations in level of arousal and in the associated mood , drive and motivation .
	manualset3
245032	3	422283	7	NULL	NULL	0	NULL	rapid fluctuations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An imbalance of ascending dopaminergic tracts may drive rapid fluctuations in level of arousal and in the associated mood , drive and motivation .
	manualset3
245033	4	422283	7	NULL	NULL	0	NULL	level of arousal 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An imbalance of ascending dopaminergic tracts may drive rapid fluctuations in level of arousal and in the associated mood , drive and motivation .
	manualset3
245034	5	422283	7	NULL	NULL	0	NULL	mood	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An imbalance of ascending dopaminergic tracts may drive rapid fluctuations in level of arousal and in the associated mood , drive and motivation .
	manualset3
245035	6	422283	7	NULL	NULL	0	NULL	drive	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An imbalance of ascending dopaminergic tracts may drive rapid fluctuations in level of arousal and in the associated mood , drive and motivation .
	manualset3
245036	7	422283	7	NULL	NULL	0	NULL	motivation	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An imbalance of ascending dopaminergic tracts may drive rapid fluctuations in level of arousal and in the associated mood , drive and motivation .
	manualset3
245037	1	422284	7	NULL	NULL	0	NULL	Symptomatic treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Symptomatic treatment of renal acidosis by oral administration of THAM citrate ) .
	manualset3
245038	2	422284	7	NULL	NULL	0	NULL	renal acidosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Symptomatic treatment of renal acidosis by oral administration of THAM citrate ) .
	manualset3
245039	3	422284	7	NULL	NULL	0	NULL	oral administration 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Symptomatic treatment of renal acidosis by oral administration of THAM citrate ) .
	manualset3
245040	4	422284	7	NULL	NULL	0	NULL	THAM citrate	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Symptomatic treatment of renal acidosis by oral administration of THAM citrate ) .
	manualset3
245041	1	422285	7	NULL	NULL	0	NULL	Layers fed diets 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Layers fed diets containing amaranth required significantly less feed to produce a dozen eggs or a gram of egg than those fed the control diet .
	manualset3
245042	2	422285	7	NULL	NULL	0	NULL	amaranth	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Layers fed diets containing amaranth required significantly less feed to produce a dozen eggs or a gram of egg than those fed the control diet .
	manualset3
245043	3	422285	7	NULL	NULL	NULL	NULL	dozen eggs	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Layers fed diets containing amaranth required significantly less feed to produce a dozen eggs or a gram of egg than those fed the control diet .
	manualset3
245044	4	422285	7	NULL	NULL	0	NULL	 gram	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Layers fed diets containing amaranth required significantly less feed to produce a dozen eggs or a gram of egg than those fed the control diet .
	manualset3
245045	5	422285	7	NULL	NULL	0	NULL	egg	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Layers fed diets containing amaranth required significantly less feed to produce a dozen eggs or a gram of egg than those fed the control diet .
	manualset3
245046	6	422285	7	NULL	NULL	0	NULL	 control diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Layers fed diets containing amaranth required significantly less feed to produce a dozen eggs or a gram of egg than those fed the control diet .
	manualset3
245047	1	422286	7	NULL	NULL	0	NULL	High-risk behavior	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	High-risk behavior in teens : self-destructive or adaptive ?
	manualset3
245048	2	422286	7	NULL	NULL	0	NULL	teens	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	High-risk behavior in teens : self-destructive or adaptive ?
	manualset3
245049	1	422287	7	NULL	NULL	0	NULL	great strength	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The great strength of the thin side of the blood-gas barrier can be attributed to the extracellular matrix , especially the type IV collagen which is predominantly located in the very thin lamina densa .
	manualset3
245050	2	422287	7	NULL	NULL	0	NULL	thin side	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The great strength of the thin side of the blood-gas barrier can be attributed to the extracellular matrix , especially the type IV collagen which is predominantly located in the very thin lamina densa .
	manualset3
245051	3	422287	7	NULL	NULL	0	NULL	blood-gas barrier	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The great strength of the thin side of the blood-gas barrier can be attributed to the extracellular matrix , especially the type IV collagen which is predominantly located in the very thin lamina densa .
	manualset3
245052	4	422287	7	NULL	NULL	0	NULL	extracellular matrix 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The great strength of the thin side of the blood-gas barrier can be attributed to the extracellular matrix , especially the type IV collagen which is predominantly located in the very thin lamina densa .
	manualset3
245053	5	422287	7	NULL	NULL	0	NULL	type IV collagen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The great strength of the thin side of the blood-gas barrier can be attributed to the extracellular matrix , especially the type IV collagen which is predominantly located in the very thin lamina densa .
	manualset3
245054	6	422287	7	NULL	NULL	0	NULL	 thin lamina densa	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The great strength of the thin side of the blood-gas barrier can be attributed to the extracellular matrix , especially the type IV collagen which is predominantly located in the very thin lamina densa .
	manualset3
245055	1	422288	7	NULL	NULL	0	NULL	relevant terms 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It also appears prudent to explain relevant terms such as ` off-label ' and ` level of evidence ' .
	manualset3
245056	2	422288	7	NULL	NULL	0	NULL	 ` off-label ' 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	It also appears prudent to explain relevant terms such as ` off-label ' and ` level of evidence ' .
	manualset3
245057	3	422288	7	NULL	NULL	0	NULL	` level of evidence '	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	It also appears prudent to explain relevant terms such as ` off-label ' and ` level of evidence ' .
	manualset3
245058	1	422289	7	NULL	NULL	0	NULL	Expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression and characterization of human D4 dopamine receptors in baculovirus-infected insect cells .
	manualset3
245059	2	422289	7	NULL	NULL	0	NULL	characterization 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression and characterization of human D4 dopamine receptors in baculovirus-infected insect cells .
	manualset3
245060	3	422289	7	NULL	NULL	0	NULL	human D4 dopamine receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression and characterization of human D4 dopamine receptors in baculovirus-infected insect cells .
	manualset3
245061	4	422289	7	NULL	NULL	0	NULL	 baculovirus-infected insect cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Expression and characterization of human D4 dopamine receptors in baculovirus-infected insect cells .
	manualset3
245062	1	422290	7	NULL	NULL	0	NULL	safety 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we evaluate the safety of IA neural progenitor cell ( NPC ) delivery to the brain .
	manualset3
245063	2	422290	7	NULL	NULL	0	NULL	IA neural progenitor cell ( NPC ) delivery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we evaluate the safety of IA neural progenitor cell ( NPC ) delivery to the brain .
	manualset3
245064	3	422290	7	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Here we evaluate the safety of IA neural progenitor cell ( NPC ) delivery to the brain .
	manualset3
245065	1	422291	7	NULL	NULL	0	NULL	immune response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An immune response to cancer is elicited in humans , as demonstrated , in part , by the identification of autoantibodies against a number of tumor-associated antigen ( TAAs ) in sera from patients with different types of cancer .
	manualset3
245066	2	422291	7	NULL	NULL	0	NULL	cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	An immune response to cancer is elicited in humans , as demonstrated , in part , by the identification of autoantibodies against a number of tumor-associated antigen ( TAAs ) in sera from patients with different types of cancer .
	manualset3
245067	3	422291	7	NULL	NULL	0	NULL	humans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	An immune response to cancer is elicited in humans , as demonstrated , in part , by the identification of autoantibodies against a number of tumor-associated antigen ( TAAs ) in sera from patients with different types of cancer .
	manualset3
245068	4	422291	7	NULL	NULL	0	NULL	identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An immune response to cancer is elicited in humans , as demonstrated , in part , by the identification of autoantibodies against a number of tumor-associated antigen ( TAAs ) in sera from patients with different types of cancer .
	manualset3
245069	5	422291	7	NULL	NULL	0	NULL	autoantibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	An immune response to cancer is elicited in humans , as demonstrated , in part , by the identification of autoantibodies against a number of tumor-associated antigen ( TAAs ) in sera from patients with different types of cancer .
	manualset3
245070	6	422291	7	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An immune response to cancer is elicited in humans , as demonstrated , in part , by the identification of autoantibodies against a number of tumor-associated antigen ( TAAs ) in sera from patients with different types of cancer .
	manualset3
245071	7	422291	7	NULL	NULL	0	NULL	tumor-associated antigen ( TAAs )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	An immune response to cancer is elicited in humans , as demonstrated , in part , by the identification of autoantibodies against a number of tumor-associated antigen ( TAAs ) in sera from patients with different types of cancer .
	manualset3
245072	8	422291	7	NULL	NULL	0	NULL	sera	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An immune response to cancer is elicited in humans , as demonstrated , in part , by the identification of autoantibodies against a number of tumor-associated antigen ( TAAs ) in sera from patients with different types of cancer .
	manualset3
245073	9	422291	7	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	An immune response to cancer is elicited in humans , as demonstrated , in part , by the identification of autoantibodies against a number of tumor-associated antigen ( TAAs ) in sera from patients with different types of cancer .
	manualset3
245074	10	422291	7	NULL	NULL	0	NULL	 different types	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	An immune response to cancer is elicited in humans , as demonstrated , in part , by the identification of autoantibodies against a number of tumor-associated antigen ( TAAs ) in sera from patients with different types of cancer .
	manualset3
245075	11	422291	7	NULL	NULL	0	NULL	cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	An immune response to cancer is elicited in humans , as demonstrated , in part , by the identification of autoantibodies against a number of tumor-associated antigen ( TAAs ) in sera from patients with different types of cancer .
	manualset3
245076	1	422292	7	NULL	NULL	0	NULL	cell line NIT-1	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The cell line NIT-1 responded to the interleukin ( IL ) -1 beta + interferon ( IFN ) - gamma stimulus with translocation of Fas to the cell surface .
	manualset3
245077	2	422292	7	NULL	NULL	NULL	NULL	interleukin ( IL ) -1 beta + interferon ( IFN ) - gamma stimulus	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The cell line NIT-1 responded to the interleukin ( IL ) -1 beta + interferon ( IFN ) - gamma stimulus with translocation of Fas to the cell surface .
	manualset3
245078	3	422292	7	NULL	NULL	0	NULL	translocation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cell line NIT-1 responded to the interleukin ( IL ) -1 beta + interferon ( IFN ) - gamma stimulus with translocation of Fas to the cell surface .
	manualset3
245079	4	422292	7	NULL	NULL	0	NULL	Fas	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The cell line NIT-1 responded to the interleukin ( IL ) -1 beta + interferon ( IFN ) - gamma stimulus with translocation of Fas to the cell surface .
	manualset3
245080	5	422292	7	NULL	NULL	0	NULL	cell surface	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The cell line NIT-1 responded to the interleukin ( IL ) -1 beta + interferon ( IFN ) - gamma stimulus with translocation of Fas to the cell surface .
	manualset3
245081	1	422293	7	NULL	NULL	0	NULL	 thickness	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The thickness of the intrapulmonary myocardial layer in the tunica adventitia of the venous wall depends on the body mass of the animal .
	manualset3
245082	2	422293	7	NULL	NULL	0	NULL	intrapulmonary myocardial layer 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The thickness of the intrapulmonary myocardial layer in the tunica adventitia of the venous wall depends on the body mass of the animal .
	manualset3
245083	3	422293	7	NULL	NULL	0	NULL	tunica adventitia	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The thickness of the intrapulmonary myocardial layer in the tunica adventitia of the venous wall depends on the body mass of the animal .
	manualset3
245084	4	422293	7	NULL	NULL	0	NULL	venous wall	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The thickness of the intrapulmonary myocardial layer in the tunica adventitia of the venous wall depends on the body mass of the animal .
	manualset3
245085	5	422293	7	NULL	NULL	0	NULL	body mass	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The thickness of the intrapulmonary myocardial layer in the tunica adventitia of the venous wall depends on the body mass of the animal .
	manualset3
245086	6	422293	7	NULL	NULL	0	NULL	animal 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The thickness of the intrapulmonary myocardial layer in the tunica adventitia of the venous wall depends on the body mass of the animal .
	manualset3
245087	1	422294	7	NULL	NULL	0	NULL	LEAFY expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	LEAFY expression procedes expression of the homeotic genes AGAMOUS and APETALA3 , which specify organ identify within the flower .
	manualset3
245088	2	422294	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	LEAFY expression procedes expression of the homeotic genes AGAMOUS and APETALA3 , which specify organ identify within the flower .
	manualset3
245089	3	422294	7	NULL	NULL	0	NULL	homeotic genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	LEAFY expression procedes expression of the homeotic genes AGAMOUS and APETALA3 , which specify organ identify within the flower .
	manualset3
245090	4	422294	7	NULL	NULL	0	NULL	AGAMOUS	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	LEAFY expression procedes expression of the homeotic genes AGAMOUS and APETALA3 , which specify organ identify within the flower .
	manualset3
245091	5	422294	7	NULL	NULL	0	NULL	APETALA3	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	LEAFY expression procedes expression of the homeotic genes AGAMOUS and APETALA3 , which specify organ identify within the flower .
	manualset3
245092	6	422294	7	NULL	NULL	0	NULL	organ	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	LEAFY expression procedes expression of the homeotic genes AGAMOUS and APETALA3 , which specify organ identify within the flower .
	manualset3
245093	7	422294	7	NULL	NULL	0	NULL	flower	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	LEAFY expression procedes expression of the homeotic genes AGAMOUS and APETALA3 , which specify organ identify within the flower .
	manualset3
245094	1	422295	7	NULL	NULL	NULL	NULL	 triclosan	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because triclosan , an antimicrobial agent included in personal care products , potentially presents high relative risk among antimicrobial agents to aquatic plants and algae , we performed laboratory experiments with the model aquatic macrophyte Lemna gibba across a gradient of environmentally relevant N : P levels with and without triclosan co-exposure .
	manualset3
245095	2	422295	7	NULL	NULL	NULL	NULL	antimicrobial agent	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because triclosan , an antimicrobial agent included in personal care products , potentially presents high relative risk among antimicrobial agents to aquatic plants and algae , we performed laboratory experiments with the model aquatic macrophyte Lemna gibba across a gradient of environmentally relevant N : P levels with and without triclosan co-exposure .
	manualset3
245096	3	422295	7	NULL	NULL	0	NULL	personal care products	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Because triclosan , an antimicrobial agent included in personal care products , potentially presents high relative risk among antimicrobial agents to aquatic plants and algae , we performed laboratory experiments with the model aquatic macrophyte Lemna gibba across a gradient of environmentally relevant N : P levels with and without triclosan co-exposure .
	manualset3
245097	4	422295	7	NULL	NULL	0	NULL	high relative risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Because triclosan , an antimicrobial agent included in personal care products , potentially presents high relative risk among antimicrobial agents to aquatic plants and algae , we performed laboratory experiments with the model aquatic macrophyte Lemna gibba across a gradient of environmentally relevant N : P levels with and without triclosan co-exposure .
	manualset3
245098	5	422295	7	NULL	NULL	0	NULL	antimicrobial agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Because triclosan , an antimicrobial agent included in personal care products , potentially presents high relative risk among antimicrobial agents to aquatic plants and algae , we performed laboratory experiments with the model aquatic macrophyte Lemna gibba across a gradient of environmentally relevant N : P levels with and without triclosan co-exposure .
	manualset3
245099	6	422295	7	NULL	NULL	0	NULL	aquatic plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Because triclosan , an antimicrobial agent included in personal care products , potentially presents high relative risk among antimicrobial agents to aquatic plants and algae , we performed laboratory experiments with the model aquatic macrophyte Lemna gibba across a gradient of environmentally relevant N : P levels with and without triclosan co-exposure .
	manualset3
245100	7	422295	7	NULL	NULL	0	NULL	algae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Because triclosan , an antimicrobial agent included in personal care products , potentially presents high relative risk among antimicrobial agents to aquatic plants and algae , we performed laboratory experiments with the model aquatic macrophyte Lemna gibba across a gradient of environmentally relevant N : P levels with and without triclosan co-exposure .
	manualset3
245101	8	422295	7	NULL	NULL	0	NULL	laboratory experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Because triclosan , an antimicrobial agent included in personal care products , potentially presents high relative risk among antimicrobial agents to aquatic plants and algae , we performed laboratory experiments with the model aquatic macrophyte Lemna gibba across a gradient of environmentally relevant N : P levels with and without triclosan co-exposure .
	manualset3
245102	9	422295	7	NULL	NULL	0	NULL	model aquatic macrophyte	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Because triclosan , an antimicrobial agent included in personal care products , potentially presents high relative risk among antimicrobial agents to aquatic plants and algae , we performed laboratory experiments with the model aquatic macrophyte Lemna gibba across a gradient of environmentally relevant N : P levels with and without triclosan co-exposure .
	manualset3
245103	10	422295	7	NULL	NULL	0	NULL	Lemna gibba	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Because triclosan , an antimicrobial agent included in personal care products , potentially presents high relative risk among antimicrobial agents to aquatic plants and algae , we performed laboratory experiments with the model aquatic macrophyte Lemna gibba across a gradient of environmentally relevant N : P levels with and without triclosan co-exposure .
	manualset3
245104	11	422295	7	NULL	NULL	0	NULL	gradient	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Because triclosan , an antimicrobial agent included in personal care products , potentially presents high relative risk among antimicrobial agents to aquatic plants and algae , we performed laboratory experiments with the model aquatic macrophyte Lemna gibba across a gradient of environmentally relevant N : P levels with and without triclosan co-exposure .
	manualset3
245105	12	422295	7	NULL	NULL	0	NULL	environmentally relevant N : P levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Because triclosan , an antimicrobial agent included in personal care products , potentially presents high relative risk among antimicrobial agents to aquatic plants and algae , we performed laboratory experiments with the model aquatic macrophyte Lemna gibba across a gradient of environmentally relevant N : P levels with and without triclosan co-exposure .
	manualset3
245106	13	422295	7	NULL	NULL	0	NULL	triclosan co-exposure 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Because triclosan , an antimicrobial agent included in personal care products , potentially presents high relative risk among antimicrobial agents to aquatic plants and algae , we performed laboratory experiments with the model aquatic macrophyte Lemna gibba across a gradient of environmentally relevant N : P levels with and without triclosan co-exposure .
	manualset3
245107	1	422296	7	NULL	NULL	0	NULL	exoantigen test reagents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We have developed exoantigen test reagents capable of identifying non-sporulating isolates of A. elegans and S. vasiformis .
	manualset3
245108	2	422296	7	NULL	NULL	0	NULL	non-sporulating isolates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We have developed exoantigen test reagents capable of identifying non-sporulating isolates of A. elegans and S. vasiformis .
	manualset3
245109	3	422296	7	NULL	NULL	0	NULL	A. elegans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We have developed exoantigen test reagents capable of identifying non-sporulating isolates of A. elegans and S. vasiformis .
	manualset3
245110	4	422296	7	NULL	NULL	0	NULL	S. vasiformis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We have developed exoantigen test reagents capable of identifying non-sporulating isolates of A. elegans and S. vasiformis .
	manualset3
245111	1	422297	7	NULL	NULL	0	NULL	mechanics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Independently of mechanics , calcifications and attachment molecules contribute to enhance vessel wall stiffness through changes in collagen cross-links , proteoglycans , integrins , and fibronectin .
	manualset3
245112	2	422297	7	NULL	NULL	0	NULL	calcifications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Independently of mechanics , calcifications and attachment molecules contribute to enhance vessel wall stiffness through changes in collagen cross-links , proteoglycans , integrins , and fibronectin .
	manualset3
245113	3	422297	7	NULL	NULL	0	NULL	attachment molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Independently of mechanics , calcifications and attachment molecules contribute to enhance vessel wall stiffness through changes in collagen cross-links , proteoglycans , integrins , and fibronectin .
	manualset3
245114	4	422297	7	NULL	NULL	0	NULL	vessel wall stiffness	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Independently of mechanics , calcifications and attachment molecules contribute to enhance vessel wall stiffness through changes in collagen cross-links , proteoglycans , integrins , and fibronectin .
	manualset3
245115	5	422297	7	NULL	NULL	0	NULL	changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Independently of mechanics , calcifications and attachment molecules contribute to enhance vessel wall stiffness through changes in collagen cross-links , proteoglycans , integrins , and fibronectin .
	manualset3
245116	6	422297	7	NULL	NULL	0	NULL	collagen cross-links	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Independently of mechanics , calcifications and attachment molecules contribute to enhance vessel wall stiffness through changes in collagen cross-links , proteoglycans , integrins , and fibronectin .
	manualset3
245117	7	422297	7	NULL	NULL	0	NULL	proteoglycans	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Independently of mechanics , calcifications and attachment molecules contribute to enhance vessel wall stiffness through changes in collagen cross-links , proteoglycans , integrins , and fibronectin .
	manualset3
245118	8	422297	7	NULL	NULL	0	NULL	 integrins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Independently of mechanics , calcifications and attachment molecules contribute to enhance vessel wall stiffness through changes in collagen cross-links , proteoglycans , integrins , and fibronectin .
	manualset3
245119	9	422297	7	NULL	NULL	0	NULL	fibronectin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Independently of mechanics , calcifications and attachment molecules contribute to enhance vessel wall stiffness through changes in collagen cross-links , proteoglycans , integrins , and fibronectin .
	manualset3
245120	1	422298	7	NULL	NULL	0	NULL	Intravenous injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous injection of STZ produced cardinal signs of diabetes mellitus including hyperglycemia , loss of body weight , polyphagia and polydipsia .
	manualset3
245121	2	422298	7	NULL	NULL	0	NULL	STZ	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous injection of STZ produced cardinal signs of diabetes mellitus including hyperglycemia , loss of body weight , polyphagia and polydipsia .
	manualset3
245122	3	422298	7	NULL	NULL	0	NULL	cardinal signs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous injection of STZ produced cardinal signs of diabetes mellitus including hyperglycemia , loss of body weight , polyphagia and polydipsia .
	manualset3
245123	4	422298	7	NULL	NULL	0	NULL	diabetes mellitus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous injection of STZ produced cardinal signs of diabetes mellitus including hyperglycemia , loss of body weight , polyphagia and polydipsia .
	manualset3
245124	5	422298	7	NULL	NULL	0	NULL	hyperglycemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous injection of STZ produced cardinal signs of diabetes mellitus including hyperglycemia , loss of body weight , polyphagia and polydipsia .
	manualset3
245125	6	422298	7	NULL	NULL	0	NULL	loss of body weight	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous injection of STZ produced cardinal signs of diabetes mellitus including hyperglycemia , loss of body weight , polyphagia and polydipsia .
	manualset3
245126	7	422298	7	NULL	NULL	0	NULL	polyphagia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous injection of STZ produced cardinal signs of diabetes mellitus including hyperglycemia , loss of body weight , polyphagia and polydipsia .
	manualset3
245127	8	422298	7	NULL	NULL	0	NULL	polydipsia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Intravenous injection of STZ produced cardinal signs of diabetes mellitus including hyperglycemia , loss of body weight , polyphagia and polydipsia .
	manualset3
245128	1	422299	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , an in vitro induction experiment was conducted using susceptible C. jejuni strain and erythromycin as a selecting agent to obtain Ery-resistant mutant with 23S rRNA gene mutation ( A2074C ) .
	manualset3
245129	2	422299	7	NULL	NULL	0	NULL	 in vitro induction experiment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , an in vitro induction experiment was conducted using susceptible C. jejuni strain and erythromycin as a selecting agent to obtain Ery-resistant mutant with 23S rRNA gene mutation ( A2074C ) .
	manualset3
245130	3	422299	7	NULL	NULL	0	NULL	susceptible C. jejuni strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , an in vitro induction experiment was conducted using susceptible C. jejuni strain and erythromycin as a selecting agent to obtain Ery-resistant mutant with 23S rRNA gene mutation ( A2074C ) .
	manualset3
245131	4	422299	7	NULL	NULL	0	NULL	erythromycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , an in vitro induction experiment was conducted using susceptible C. jejuni strain and erythromycin as a selecting agent to obtain Ery-resistant mutant with 23S rRNA gene mutation ( A2074C ) .
	manualset3
245132	5	422299	7	NULL	NULL	0	NULL	selecting agent 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , an in vitro induction experiment was conducted using susceptible C. jejuni strain and erythromycin as a selecting agent to obtain Ery-resistant mutant with 23S rRNA gene mutation ( A2074C ) .
	manualset3
245133	6	422299	7	NULL	NULL	0	NULL	Ery-resistant mutant	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , an in vitro induction experiment was conducted using susceptible C. jejuni strain and erythromycin as a selecting agent to obtain Ery-resistant mutant with 23S rRNA gene mutation ( A2074C ) .
	manualset3
245134	7	422299	7	NULL	NULL	0	NULL	23S rRNA gene mutation ( A2074C )	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this study , an in vitro induction experiment was conducted using susceptible C. jejuni strain and erythromycin as a selecting agent to obtain Ery-resistant mutant with 23S rRNA gene mutation ( A2074C ) .
	manualset3
245135	1	422300	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that there is a high concentration of acrylamide in precooked , battered protein foods and that the concentration changes considerably during storage , which may lead to almost twice the initial amounts when air is present within the package .
	manualset3
245136	2	422300	7	NULL	NULL	0	NULL	high concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that there is a high concentration of acrylamide in precooked , battered protein foods and that the concentration changes considerably during storage , which may lead to almost twice the initial amounts when air is present within the package .
	manualset3
245137	3	422300	7	NULL	NULL	0	NULL	acrylamide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that there is a high concentration of acrylamide in precooked , battered protein foods and that the concentration changes considerably during storage , which may lead to almost twice the initial amounts when air is present within the package .
	manualset3
245138	4	422300	7	NULL	NULL	0	NULL	battered protein foods	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that there is a high concentration of acrylamide in precooked , battered protein foods and that the concentration changes considerably during storage , which may lead to almost twice the initial amounts when air is present within the package .
	manualset3
245139	5	422300	7	NULL	NULL	0	NULL	 concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that there is a high concentration of acrylamide in precooked , battered protein foods and that the concentration changes considerably during storage , which may lead to almost twice the initial amounts when air is present within the package .
	manualset3
245140	6	422300	7	NULL	NULL	0	NULL	storage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that there is a high concentration of acrylamide in precooked , battered protein foods and that the concentration changes considerably during storage , which may lead to almost twice the initial amounts when air is present within the package .
	manualset3
245141	7	422300	7	NULL	NULL	0	NULL	 initial amounts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that there is a high concentration of acrylamide in precooked , battered protein foods and that the concentration changes considerably during storage , which may lead to almost twice the initial amounts when air is present within the package .
	manualset3
245142	8	422300	7	NULL	NULL	0	NULL	air	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that there is a high concentration of acrylamide in precooked , battered protein foods and that the concentration changes considerably during storage , which may lead to almost twice the initial amounts when air is present within the package .
	manualset3
245143	9	422300	7	NULL	NULL	0	NULL	package	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	These data indicate that there is a high concentration of acrylamide in precooked , battered protein foods and that the concentration changes considerably during storage , which may lead to almost twice the initial amounts when air is present within the package .
	manualset3
245144	1	422301	7	NULL	NULL	0	NULL	losses	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such losses might counterbalace the calcium gained by intestinal absorption ( about 4-5 mmol/day or 160-200 mg/day in patients with an oral daily calcium intake of 1-1 .5 g and normal vitamin D status ) and ensure an overall approximately neutral calcium balance .
	manualset3
245145	2	422301	7	NULL	NULL	0	NULL	calcium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Such losses might counterbalace the calcium gained by intestinal absorption ( about 4-5 mmol/day or 160-200 mg/day in patients with an oral daily calcium intake of 1-1 .5 g and normal vitamin D status ) and ensure an overall approximately neutral calcium balance .
	manualset3
245146	3	422301	7	NULL	NULL	0	NULL	intestinal absorption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such losses might counterbalace the calcium gained by intestinal absorption ( about 4-5 mmol/day or 160-200 mg/day in patients with an oral daily calcium intake of 1-1 .5 g and normal vitamin D status ) and ensure an overall approximately neutral calcium balance .
	manualset3
245147	4	422301	7	NULL	NULL	0	NULL	4-5 mmol/day	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Such losses might counterbalace the calcium gained by intestinal absorption ( about 4-5 mmol/day or 160-200 mg/day in patients with an oral daily calcium intake of 1-1 .5 g and normal vitamin D status ) and ensure an overall approximately neutral calcium balance .
	manualset3
245148	5	422301	7	NULL	NULL	0	NULL	160-200 mg/day	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Such losses might counterbalace the calcium gained by intestinal absorption ( about 4-5 mmol/day or 160-200 mg/day in patients with an oral daily calcium intake of 1-1 .5 g and normal vitamin D status ) and ensure an overall approximately neutral calcium balance .
	manualset3
245149	6	422301	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Such losses might counterbalace the calcium gained by intestinal absorption ( about 4-5 mmol/day or 160-200 mg/day in patients with an oral daily calcium intake of 1-1 .5 g and normal vitamin D status ) and ensure an overall approximately neutral calcium balance .
	manualset3
245150	7	422301	7	NULL	NULL	0	NULL	oral daily calcium intake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Such losses might counterbalace the calcium gained by intestinal absorption ( about 4-5 mmol/day or 160-200 mg/day in patients with an oral daily calcium intake of 1-1 .5 g and normal vitamin D status ) and ensure an overall approximately neutral calcium balance .
	manualset3
245151	8	422301	7	NULL	NULL	0	NULL	1-1 .5 g	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Such losses might counterbalace the calcium gained by intestinal absorption ( about 4-5 mmol/day or 160-200 mg/day in patients with an oral daily calcium intake of 1-1 .5 g and normal vitamin D status ) and ensure an overall approximately neutral calcium balance .
	manualset3
245152	9	422301	7	NULL	NULL	0	NULL	normal vitamin D status 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Such losses might counterbalace the calcium gained by intestinal absorption ( about 4-5 mmol/day or 160-200 mg/day in patients with an oral daily calcium intake of 1-1 .5 g and normal vitamin D status ) and ensure an overall approximately neutral calcium balance .
	manualset3
245153	10	422301	7	NULL	NULL	0	NULL	neutral calcium balance 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Such losses might counterbalace the calcium gained by intestinal absorption ( about 4-5 mmol/day or 160-200 mg/day in patients with an oral daily calcium intake of 1-1 .5 g and normal vitamin D status ) and ensure an overall approximately neutral calcium balance .
	manualset3
245154	1	422302	7	NULL	NULL	0	NULL	Diaphragmatic hernias	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Diaphragmatic hernias and anemias ) .
	manualset3
245155	2	422302	7	NULL	NULL	0	NULL	anemias	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Diaphragmatic hernias and anemias ) .
	manualset3
245156	1	422303	7	NULL	NULL	0	NULL	immunoassay based technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	An immunoassay based technique is used for the detection of psychoactive substances in the sweat deposited within fingermarks of a narcotic drug user .
	manualset3
245157	2	422303	7	NULL	NULL	0	NULL	detection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An immunoassay based technique is used for the detection of psychoactive substances in the sweat deposited within fingermarks of a narcotic drug user .
	manualset3
245158	3	422303	7	NULL	NULL	0	NULL	psychoactive substances	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	An immunoassay based technique is used for the detection of psychoactive substances in the sweat deposited within fingermarks of a narcotic drug user .
	manualset3
245159	4	422303	7	NULL	NULL	0	NULL	sweat	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	An immunoassay based technique is used for the detection of psychoactive substances in the sweat deposited within fingermarks of a narcotic drug user .
	manualset3
245160	5	422303	7	NULL	NULL	0	NULL	fingermarks	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An immunoassay based technique is used for the detection of psychoactive substances in the sweat deposited within fingermarks of a narcotic drug user .
	manualset3
245161	6	422303	7	NULL	NULL	0	NULL	narcotic drug user	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	An immunoassay based technique is used for the detection of psychoactive substances in the sweat deposited within fingermarks of a narcotic drug user .
	manualset3
245162	1	422304	7	NULL	NULL	0	NULL	 iron overload	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This reflects iron overload due to blood transfusions given to treat renal anemia .
	manualset3
245163	2	422304	7	NULL	NULL	0	NULL	blood transfusions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	This reflects iron overload due to blood transfusions given to treat renal anemia .
	manualset3
245164	3	422304	7	NULL	NULL	0	NULL	renal anemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	This reflects iron overload due to blood transfusions given to treat renal anemia .
	manualset3
245165	1	422305	7	NULL	NULL	0	NULL	serum -free B6 ES cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We newly established serum - and feeder-free B6 ES cells with full developmental potential by using leukemia inhibitory factor ( LIF ) and 6-bromoindirubin-3 ' - oxime ( BIO ) , a glycogen synthase kinase-3 ( GSK3 ) inhibitor .
	manualset3
245166	2	422305	7	NULL	NULL	0	NULL	feeder-free B6 ES cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	We newly established serum - and feeder-free B6 ES cells with full developmental potential by using leukemia inhibitory factor ( LIF ) and 6-bromoindirubin-3 ' - oxime ( BIO ) , a glycogen synthase kinase-3 ( GSK3 ) inhibitor .
	manualset3
245167	3	422305	7	NULL	NULL	0	NULL	full developmental potential	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We newly established serum - and feeder-free B6 ES cells with full developmental potential by using leukemia inhibitory factor ( LIF ) and 6-bromoindirubin-3 ' - oxime ( BIO ) , a glycogen synthase kinase-3 ( GSK3 ) inhibitor .
	manualset3
245168	4	422305	7	NULL	NULL	0	NULL	leukemia inhibitory factor ( LIF ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	We newly established serum - and feeder-free B6 ES cells with full developmental potential by using leukemia inhibitory factor ( LIF ) and 6-bromoindirubin-3 ' - oxime ( BIO ) , a glycogen synthase kinase-3 ( GSK3 ) inhibitor .
	manualset3
245169	5	422305	7	NULL	NULL	0	NULL	6-bromoindirubin-3 ' - oxime ( BIO ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We newly established serum - and feeder-free B6 ES cells with full developmental potential by using leukemia inhibitory factor ( LIF ) and 6-bromoindirubin-3 ' - oxime ( BIO ) , a glycogen synthase kinase-3 ( GSK3 ) inhibitor .
	manualset3
245170	6	422305	7	NULL	NULL	0	NULL	glycogen synthase kinase-3 ( GSK3 ) inhibitor 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We newly established serum - and feeder-free B6 ES cells with full developmental potential by using leukemia inhibitory factor ( LIF ) and 6-bromoindirubin-3 ' - oxime ( BIO ) , a glycogen synthase kinase-3 ( GSK3 ) inhibitor .
	manualset3
245171	1	422306	7	NULL	NULL	0	NULL	Study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Study of a reversible stage in the thermodenaturation of bovine beta-lactoglobulin A ) .
	manualset3
245172	2	422306	7	NULL	NULL	0	NULL	 reversible stage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Study of a reversible stage in the thermodenaturation of bovine beta-lactoglobulin A ) .
	manualset3
245173	3	422306	7	NULL	NULL	0	NULL	thermodenaturation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Study of a reversible stage in the thermodenaturation of bovine beta-lactoglobulin A ) .
	manualset3
245174	4	422306	7	NULL	NULL	0	NULL	bovine beta-lactoglobulin A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Study of a reversible stage in the thermodenaturation of bovine beta-lactoglobulin A ) .
	manualset3
245175	1	422307	7	NULL	NULL	0	NULL	primary screening	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Following primary screening by ELISA , the binding of the MAbs to the native form of human TF was demonstrated in flow cytometry using a stable cell line expressing human TF .
	manualset3
245176	2	422307	7	NULL	NULL	0	NULL	ELISA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Following primary screening by ELISA , the binding of the MAbs to the native form of human TF was demonstrated in flow cytometry using a stable cell line expressing human TF .
	manualset3
245177	3	422307	7	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Following primary screening by ELISA , the binding of the MAbs to the native form of human TF was demonstrated in flow cytometry using a stable cell line expressing human TF .
	manualset3
245178	4	422307	7	NULL	NULL	0	NULL	MAbs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Following primary screening by ELISA , the binding of the MAbs to the native form of human TF was demonstrated in flow cytometry using a stable cell line expressing human TF .
	manualset3
245179	5	422307	7	NULL	NULL	0	NULL	 native form 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Following primary screening by ELISA , the binding of the MAbs to the native form of human TF was demonstrated in flow cytometry using a stable cell line expressing human TF .
	manualset3
245180	6	422307	7	NULL	NULL	0	NULL	human TF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Following primary screening by ELISA , the binding of the MAbs to the native form of human TF was demonstrated in flow cytometry using a stable cell line expressing human TF .
	manualset3
245181	7	422307	7	NULL	NULL	0	NULL	flow cytometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Following primary screening by ELISA , the binding of the MAbs to the native form of human TF was demonstrated in flow cytometry using a stable cell line expressing human TF .
	manualset3
245182	8	422307	7	NULL	NULL	0	NULL	 stable cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Following primary screening by ELISA , the binding of the MAbs to the native form of human TF was demonstrated in flow cytometry using a stable cell line expressing human TF .
	manualset3
245183	9	422307	7	NULL	NULL	0	NULL	human TF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Following primary screening by ELISA , the binding of the MAbs to the native form of human TF was demonstrated in flow cytometry using a stable cell line expressing human TF .
	manualset3
245184	1	422308	7	NULL	NULL	0	NULL	 study periods	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	During the study periods , the number of patients receiving medical treatment related to osteoporosis increased from 1 , 034 , 399 to 1 , 392 , 189 for women and from 120 , 496 to 171 , 902 for men .
	manualset3
245185	2	422308	7	NULL	NULL	0	NULL	 number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	During the study periods , the number of patients receiving medical treatment related to osteoporosis increased from 1 , 034 , 399 to 1 , 392 , 189 for women and from 120 , 496 to 171 , 902 for men .
	manualset3
245186	3	422308	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	During the study periods , the number of patients receiving medical treatment related to osteoporosis increased from 1 , 034 , 399 to 1 , 392 , 189 for women and from 120 , 496 to 171 , 902 for men .
	manualset3
245187	4	422308	7	NULL	NULL	0	NULL	medical treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	During the study periods , the number of patients receiving medical treatment related to osteoporosis increased from 1 , 034 , 399 to 1 , 392 , 189 for women and from 120 , 496 to 171 , 902 for men .
	manualset3
245188	5	422308	7	NULL	NULL	0	NULL	osteoporosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	During the study periods , the number of patients receiving medical treatment related to osteoporosis increased from 1 , 034 , 399 to 1 , 392 , 189 for women and from 120 , 496 to 171 , 902 for men .
	manualset3
245189	6	422308	7	NULL	NULL	NULL	NULL	1 , 034 , 399 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the study periods , the number of patients receiving medical treatment related to osteoporosis increased from 1 , 034 , 399 to 1 , 392 , 189 for women and from 120 , 496 to 171 , 902 for men .
	manualset3
245190	7	422308	7	NULL	NULL	NULL	NULL	 1 , 392 , 189	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the study periods , the number of patients receiving medical treatment related to osteoporosis increased from 1 , 034 , 399 to 1 , 392 , 189 for women and from 120 , 496 to 171 , 902 for men .
	manualset3
245191	8	422308	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	During the study periods , the number of patients receiving medical treatment related to osteoporosis increased from 1 , 034 , 399 to 1 , 392 , 189 for women and from 120 , 496 to 171 , 902 for men .
	manualset3
245192	9	422308	7	NULL	NULL	0	NULL	120 , 496	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During the study periods , the number of patients receiving medical treatment related to osteoporosis increased from 1 , 034 , 399 to 1 , 392 , 189 for women and from 120 , 496 to 171 , 902 for men .
	manualset3
245193	10	422308	7	NULL	NULL	0	NULL	171 , 902	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During the study periods , the number of patients receiving medical treatment related to osteoporosis increased from 1 , 034 , 399 to 1 , 392 , 189 for women and from 120 , 496 to 171 , 902 for men .
	manualset3
245194	11	422308	7	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	During the study periods , the number of patients receiving medical treatment related to osteoporosis increased from 1 , 034 , 399 to 1 , 392 , 189 for women and from 120 , 496 to 171 , 902 for men .
	manualset3
245419	1	422309	7	NULL	NULL	0	NULL	Battered/shaken baby syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Battered/shaken baby syndrome is a clinical and pathologic diagnosis based on clinical examination , central nervous system dysfunction , and intracranial , optic nerve sheath , and retinal hemorrhages in infants under the age of three years .
	manualset3
245420	2	422309	7	NULL	NULL	0	NULL	clinical diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Battered/shaken baby syndrome is a clinical and pathologic diagnosis based on clinical examination , central nervous system dysfunction , and intracranial , optic nerve sheath , and retinal hemorrhages in infants under the age of three years .
	manualset3
245421	3	422309	7	NULL	NULL	0	NULL	pathologic diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Battered/shaken baby syndrome is a clinical and pathologic diagnosis based on clinical examination , central nervous system dysfunction , and intracranial , optic nerve sheath , and retinal hemorrhages in infants under the age of three years .
	manualset3
245422	4	422309	7	NULL	NULL	0	NULL	clinical examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Battered/shaken baby syndrome is a clinical and pathologic diagnosis based on clinical examination , central nervous system dysfunction , and intracranial , optic nerve sheath , and retinal hemorrhages in infants under the age of three years .
	manualset3
245423	5	422309	7	NULL	NULL	0	NULL	central nervous system dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Battered/shaken baby syndrome is a clinical and pathologic diagnosis based on clinical examination , central nervous system dysfunction , and intracranial , optic nerve sheath , and retinal hemorrhages in infants under the age of three years .
	manualset3
245424	6	422309	7	NULL	NULL	0	NULL	intracranial , optic nerve sheath	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Battered/shaken baby syndrome is a clinical and pathologic diagnosis based on clinical examination , central nervous system dysfunction , and intracranial , optic nerve sheath , and retinal hemorrhages in infants under the age of three years .
	manualset3
245425	7	422309	7	NULL	NULL	0	NULL	retinal hemorrhages 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Battered/shaken baby syndrome is a clinical and pathologic diagnosis based on clinical examination , central nervous system dysfunction , and intracranial , optic nerve sheath , and retinal hemorrhages in infants under the age of three years .
	manualset3
245426	8	422309	7	NULL	NULL	0	NULL	infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Battered/shaken baby syndrome is a clinical and pathologic diagnosis based on clinical examination , central nervous system dysfunction , and intracranial , optic nerve sheath , and retinal hemorrhages in infants under the age of three years .
	manualset3
245427	9	422309	7	NULL	NULL	0	NULL	age	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Battered/shaken baby syndrome is a clinical and pathologic diagnosis based on clinical examination , central nervous system dysfunction , and intracranial , optic nerve sheath , and retinal hemorrhages in infants under the age of three years .
	manualset3
245428	10	422309	7	NULL	NULL	0	NULL	three years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Battered/shaken baby syndrome is a clinical and pathologic diagnosis based on clinical examination , central nervous system dysfunction , and intracranial , optic nerve sheath , and retinal hemorrhages in infants under the age of three years .
	manualset3
245429	1	422310	7	NULL	NULL	0	NULL	BACKGROUND	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	BACKGROUND : The ionic mechanism underlying the transient inward current ( I ( ti ) ) , the current responsible for delayed afterdepolarizations ( DADs ) , appears to be different in ventricular myocytes and Purkinje fibers .
	manualset3
245430	2	422310	7	NULL	NULL	0	NULL	 ionic mechanism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	BACKGROUND : The ionic mechanism underlying the transient inward current ( I ( ti ) ) , the current responsible for delayed afterdepolarizations ( DADs ) , appears to be different in ventricular myocytes and Purkinje fibers .
	manualset3
245431	3	422310	7	NULL	NULL	0	NULL	 transient inward current ( I ( ti ) )	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	BACKGROUND : The ionic mechanism underlying the transient inward current ( I ( ti ) ) , the current responsible for delayed afterdepolarizations ( DADs ) , appears to be different in ventricular myocytes and Purkinje fibers .
	manualset3
245432	4	422310	7	NULL	NULL	0	NULL	current	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	BACKGROUND : The ionic mechanism underlying the transient inward current ( I ( ti ) ) , the current responsible for delayed afterdepolarizations ( DADs ) , appears to be different in ventricular myocytes and Purkinje fibers .
	manualset3
245433	5	422310	7	NULL	NULL	0	NULL	delayed afterdepolarizations ( DADs )	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	BACKGROUND : The ionic mechanism underlying the transient inward current ( I ( ti ) ) , the current responsible for delayed afterdepolarizations ( DADs ) , appears to be different in ventricular myocytes and Purkinje fibers .
	manualset3
245434	6	422310	7	NULL	NULL	0	NULL	ventricular myocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	BACKGROUND : The ionic mechanism underlying the transient inward current ( I ( ti ) ) , the current responsible for delayed afterdepolarizations ( DADs ) , appears to be different in ventricular myocytes and Purkinje fibers .
	manualset3
245435	7	422310	7	NULL	NULL	0	NULL	Purkinje fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	BACKGROUND : The ionic mechanism underlying the transient inward current ( I ( ti ) ) , the current responsible for delayed afterdepolarizations ( DADs ) , appears to be different in ventricular myocytes and Purkinje fibers .
	manualset3
245436	1	422311	7	NULL	NULL	0	NULL	Cardiogenic shock	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Cardiogenic shock without flow-limiting angiographic coronary artery disease : ( from the Should We Emergently Revascularize Occluded Coronary Arteries for Cardiogenic Shock Trial and Registry ) .
	manualset3
245437	2	422311	7	NULL	NULL	0	NULL	 flow-limiting angiographic coronary artery disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Cardiogenic shock without flow-limiting angiographic coronary artery disease : ( from the Should We Emergently Revascularize Occluded Coronary Arteries for Cardiogenic Shock Trial and Registry ) .
	manualset3
245438	3	422311	7	NULL	NULL	0	NULL	Occluded Coronary Arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Cardiogenic shock without flow-limiting angiographic coronary artery disease : ( from the Should We Emergently Revascularize Occluded Coronary Arteries for Cardiogenic Shock Trial and Registry ) .
	manualset3
245439	4	422311	7	NULL	NULL	0	NULL	Cardiogenic Shock Trial 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Cardiogenic shock without flow-limiting angiographic coronary artery disease : ( from the Should We Emergently Revascularize Occluded Coronary Arteries for Cardiogenic Shock Trial and Registry ) .
	manualset3
245440	5	422311	7	NULL	NULL	0	NULL	Registry	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Cardiogenic shock without flow-limiting angiographic coronary artery disease : ( from the Should We Emergently Revascularize Occluded Coronary Arteries for Cardiogenic Shock Trial and Registry ) .
	manualset3
245441	1	422312	7	NULL	NULL	0	NULL	Calcineurin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Calcineurin is a calcium-dependent , serine/threonine phosphatase that functions as a signaling intermediate .
	manualset3
245442	2	422312	7	NULL	NULL	0	NULL	 serine/threonine phosphatase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Calcineurin is a calcium-dependent , serine/threonine phosphatase that functions as a signaling intermediate .
	manualset3
245443	3	422312	7	NULL	NULL	0	NULL	signaling intermediate	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Calcineurin is a calcium-dependent , serine/threonine phosphatase that functions as a signaling intermediate .
	manualset3
245445	1	422313	7	NULL	NULL	0	NULL	One	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the four leukemic cases was clinically silent and might have escaped detection except for phenotyping .
	manualset3
245448	2	422313	7	NULL	NULL	0	NULL	 four leukemic cases 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the four leukemic cases was clinically silent and might have escaped detection except for phenotyping .
	manualset3
245450	3	422313	7	NULL	NULL	0	NULL	detection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the four leukemic cases was clinically silent and might have escaped detection except for phenotyping .
	manualset3
245452	4	422313	7	NULL	NULL	0	NULL	phenotyping 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	One of the four leukemic cases was clinically silent and might have escaped detection except for phenotyping .
	manualset3
245469	1	422314	7	NULL	NULL	0	NULL	present data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data suggest that the CD4-8 - TCR alpha beta + thymocyte population is a functional T cell lineage which may serve as cells of immune defense and/or immune regulation .
	manualset3
245470	2	422314	7	NULL	NULL	0	NULL	CD4-8 - TCR alpha beta + thymocyte population	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data suggest that the CD4-8 - TCR alpha beta + thymocyte population is a functional T cell lineage which may serve as cells of immune defense and/or immune regulation .
	manualset3
245471	3	422314	7	NULL	NULL	0	NULL	functional T cell lineage	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data suggest that the CD4-8 - TCR alpha beta + thymocyte population is a functional T cell lineage which may serve as cells of immune defense and/or immune regulation .
	manualset3
245472	4	422314	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data suggest that the CD4-8 - TCR alpha beta + thymocyte population is a functional T cell lineage which may serve as cells of immune defense and/or immune regulation .
	manualset3
245473	5	422314	7	NULL	NULL	0	NULL	immune defense	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data suggest that the CD4-8 - TCR alpha beta + thymocyte population is a functional T cell lineage which may serve as cells of immune defense and/or immune regulation .
	manualset3
245474	6	422314	7	NULL	NULL	0	NULL	immune regulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present data suggest that the CD4-8 - TCR alpha beta + thymocyte population is a functional T cell lineage which may serve as cells of immune defense and/or immune regulation .
	manualset3
245475	1	422315	7	NULL	NULL	0	NULL	immunological approach 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An immunological approach to the role of the low molecular weight subunits in myosin .
	manualset3
245476	2	422315	7	NULL	NULL	0	NULL	 role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An immunological approach to the role of the low molecular weight subunits in myosin .
	manualset3
245477	3	422315	7	NULL	NULL	0	NULL	low molecular weight subunits	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	An immunological approach to the role of the low molecular weight subunits in myosin .
	manualset3
245478	4	422315	7	NULL	NULL	0	NULL	myosin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	An immunological approach to the role of the low molecular weight subunits in myosin .
	manualset3
245479	1	422316	7	NULL	NULL	0	NULL	oestrogenic properties	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The oestrogenic and antioestrogenic properties of tamoxifen and its monohydroxylated ( monohydroxytamoxifen ) and dihydroxylated ( dihydroxytamoxifen ) metabolites have been investigated in the immature rat .
	manualset3
245480	2	422316	7	NULL	NULL	0	NULL	antioestrogenic properties	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The oestrogenic and antioestrogenic properties of tamoxifen and its monohydroxylated ( monohydroxytamoxifen ) and dihydroxylated ( dihydroxytamoxifen ) metabolites have been investigated in the immature rat .
	manualset3
245481	3	422316	7	NULL	NULL	0	NULL	tamoxifen	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The oestrogenic and antioestrogenic properties of tamoxifen and its monohydroxylated ( monohydroxytamoxifen ) and dihydroxylated ( dihydroxytamoxifen ) metabolites have been investigated in the immature rat .
	manualset3
245482	4	422316	7	NULL	NULL	0	NULL	monohydroxylated ( monohydroxytamoxifen )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The oestrogenic and antioestrogenic properties of tamoxifen and its monohydroxylated ( monohydroxytamoxifen ) and dihydroxylated ( dihydroxytamoxifen ) metabolites have been investigated in the immature rat .
	manualset3
245483	5	422316	7	NULL	NULL	0	NULL	dihydroxylated ( dihydroxytamoxifen ) metabolites	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The oestrogenic and antioestrogenic properties of tamoxifen and its monohydroxylated ( monohydroxytamoxifen ) and dihydroxylated ( dihydroxytamoxifen ) metabolites have been investigated in the immature rat .
	manualset3
245484	6	422316	7	NULL	NULL	0	NULL	immature rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The oestrogenic and antioestrogenic properties of tamoxifen and its monohydroxylated ( monohydroxytamoxifen ) and dihydroxylated ( dihydroxytamoxifen ) metabolites have been investigated in the immature rat .
	manualset3
245487	1	422317	7	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Further studies are needed to confirm if the cyt-b + COI-COII haplotypes help to assign certain phylogeographic patterns to the branch C and to clarify phylogenetic relationships among A. mellifera subspecies .
	manualset3
245489	2	422317	7	NULL	NULL	0	NULL	cyt-b + COI-COII haplotypes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Further studies are needed to confirm if the cyt-b + COI-COII haplotypes help to assign certain phylogeographic patterns to the branch C and to clarify phylogenetic relationships among A. mellifera subspecies .
	manualset3
245491	3	422317	7	NULL	NULL	0	NULL	phylogeographic patterns	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further studies are needed to confirm if the cyt-b + COI-COII haplotypes help to assign certain phylogeographic patterns to the branch C and to clarify phylogenetic relationships among A. mellifera subspecies .
	manualset3
245494	4	422317	7	NULL	NULL	0	NULL	branch C	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Further studies are needed to confirm if the cyt-b + COI-COII haplotypes help to assign certain phylogeographic patterns to the branch C and to clarify phylogenetic relationships among A. mellifera subspecies .
	manualset3
245495	5	422317	7	NULL	NULL	0	NULL	phylogenetic relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Further studies are needed to confirm if the cyt-b + COI-COII haplotypes help to assign certain phylogeographic patterns to the branch C and to clarify phylogenetic relationships among A. mellifera subspecies .
	manualset3
245497	6	422317	7	NULL	NULL	0	NULL	A. mellifera subspecies	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Further studies are needed to confirm if the cyt-b + COI-COII haplotypes help to assign certain phylogeographic patterns to the branch C and to clarify phylogenetic relationships among A. mellifera subspecies .
	manualset3
245498	1	422318	7	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of LPS was dependent on the presence of the serum protein LBP ( lipopolysaccharide-binding protein ) , as shown by the potentiating effect of human recombinant LBP or serum .
	manualset3
245499	2	422318	7	NULL	NULL	0	NULL	LPS	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of LPS was dependent on the presence of the serum protein LBP ( lipopolysaccharide-binding protein ) , as shown by the potentiating effect of human recombinant LBP or serum .
	manualset3
245500	3	422318	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of LPS was dependent on the presence of the serum protein LBP ( lipopolysaccharide-binding protein ) , as shown by the potentiating effect of human recombinant LBP or serum .
	manualset3
245501	4	422318	7	NULL	NULL	0	NULL	serum protein LBP ( lipopolysaccharide-binding protein )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of LPS was dependent on the presence of the serum protein LBP ( lipopolysaccharide-binding protein ) , as shown by the potentiating effect of human recombinant LBP or serum .
	manualset3
245502	5	422318	7	NULL	NULL	0	NULL	potentiating effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of LPS was dependent on the presence of the serum protein LBP ( lipopolysaccharide-binding protein ) , as shown by the potentiating effect of human recombinant LBP or serum .
	manualset3
245503	6	422318	7	NULL	NULL	0	NULL	human recombinant LBP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of LPS was dependent on the presence of the serum protein LBP ( lipopolysaccharide-binding protein ) , as shown by the potentiating effect of human recombinant LBP or serum .
	manualset3
245504	7	422318	7	NULL	NULL	0	NULL	serum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The effect of LPS was dependent on the presence of the serum protein LBP ( lipopolysaccharide-binding protein ) , as shown by the potentiating effect of human recombinant LBP or serum .
	manualset3
245506	1	422319	7	NULL	NULL	0	NULL	conclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This conclusion was based on the observations that purified CD38 effectively competes with p190 , its accumulation is preceded by the accumulation of CD38 , it immunoreacted with three different monospecific anti-CD38 antibodies on immunoblots , and its peptide map revealed several peptides in common with CD38 .
	manualset3
245507	2	422319	7	NULL	NULL	0	NULL	observations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This conclusion was based on the observations that purified CD38 effectively competes with p190 , its accumulation is preceded by the accumulation of CD38 , it immunoreacted with three different monospecific anti-CD38 antibodies on immunoblots , and its peptide map revealed several peptides in common with CD38 .
	manualset3
245508	3	422319	7	NULL	NULL	0	NULL	purified CD38	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	This conclusion was based on the observations that purified CD38 effectively competes with p190 , its accumulation is preceded by the accumulation of CD38 , it immunoreacted with three different monospecific anti-CD38 antibodies on immunoblots , and its peptide map revealed several peptides in common with CD38 .
	manualset3
245511	4	422319	7	NULL	NULL	0	NULL	p190	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	This conclusion was based on the observations that purified CD38 effectively competes with p190 , its accumulation is preceded by the accumulation of CD38 , it immunoreacted with three different monospecific anti-CD38 antibodies on immunoblots , and its peptide map revealed several peptides in common with CD38 .
	manualset3
245513	5	422319	7	NULL	NULL	0	NULL	accumulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This conclusion was based on the observations that purified CD38 effectively competes with p190 , its accumulation is preceded by the accumulation of CD38 , it immunoreacted with three different monospecific anti-CD38 antibodies on immunoblots , and its peptide map revealed several peptides in common with CD38 .
	manualset3
245519	6	422319	7	NULL	NULL	NULL	NULL	accumulation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	This conclusion was based on the observations that purified CD38 effectively competes with p190 , its accumulation is preceded by the accumulation of CD38 , it immunoreacted with three different monospecific anti-CD38 antibodies on immunoblots , and its peptide map revealed several peptides in common with CD38 .
	manualset3
245520	7	422319	7	NULL	NULL	0	NULL	CD38	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	This conclusion was based on the observations that purified CD38 effectively competes with p190 , its accumulation is preceded by the accumulation of CD38 , it immunoreacted with three different monospecific anti-CD38 antibodies on immunoblots , and its peptide map revealed several peptides in common with CD38 .
	manualset3
245521	8	422319	7	NULL	NULL	0	NULL	three 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	This conclusion was based on the observations that purified CD38 effectively competes with p190 , its accumulation is preceded by the accumulation of CD38 , it immunoreacted with three different monospecific anti-CD38 antibodies on immunoblots , and its peptide map revealed several peptides in common with CD38 .
	manualset3
245522	9	422319	7	NULL	NULL	0	NULL	monospecific anti-CD38 antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This conclusion was based on the observations that purified CD38 effectively competes with p190 , its accumulation is preceded by the accumulation of CD38 , it immunoreacted with three different monospecific anti-CD38 antibodies on immunoblots , and its peptide map revealed several peptides in common with CD38 .
	manualset3
245523	10	422319	7	NULL	NULL	0	NULL	immunoblots	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	This conclusion was based on the observations that purified CD38 effectively competes with p190 , its accumulation is preceded by the accumulation of CD38 , it immunoreacted with three different monospecific anti-CD38 antibodies on immunoblots , and its peptide map revealed several peptides in common with CD38 .
	manualset3
245524	11	422319	7	NULL	NULL	0	NULL	peptide map	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This conclusion was based on the observations that purified CD38 effectively competes with p190 , its accumulation is preceded by the accumulation of CD38 , it immunoreacted with three different monospecific anti-CD38 antibodies on immunoblots , and its peptide map revealed several peptides in common with CD38 .
	manualset3
245525	12	422319	7	NULL	NULL	0	NULL	several peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	This conclusion was based on the observations that purified CD38 effectively competes with p190 , its accumulation is preceded by the accumulation of CD38 , it immunoreacted with three different monospecific anti-CD38 antibodies on immunoblots , and its peptide map revealed several peptides in common with CD38 .
	manualset3
245526	13	422319	7	NULL	NULL	0	NULL	CD38	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	This conclusion was based on the observations that purified CD38 effectively competes with p190 , its accumulation is preceded by the accumulation of CD38 , it immunoreacted with three different monospecific anti-CD38 antibodies on immunoblots , and its peptide map revealed several peptides in common with CD38 .
	manualset3
245527	1	422320	7	NULL	NULL	0	NULL	perineal , one-stage bulboprostatic anastomotic operation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The contemporary , perineal , one-stage bulboprostatic anastomotic operation as popularized by Turner-Warwick ( 20 ) with selective scar excision is a versatile procedure with a high patent lumen success .
	manualset3
245528	2	422320	7	NULL	NULL	0	NULL	Turner-Warwick 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The contemporary , perineal , one-stage bulboprostatic anastomotic operation as popularized by Turner-Warwick ( 20 ) with selective scar excision is a versatile procedure with a high patent lumen success .
	manualset3
245529	3	422320	7	NULL	NULL	0	NULL	selective scar excision	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The contemporary , perineal , one-stage bulboprostatic anastomotic operation as popularized by Turner-Warwick ( 20 ) with selective scar excision is a versatile procedure with a high patent lumen success .
	manualset3
245530	4	422320	7	NULL	NULL	0	NULL	versatile procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The contemporary , perineal , one-stage bulboprostatic anastomotic operation as popularized by Turner-Warwick ( 20 ) with selective scar excision is a versatile procedure with a high patent lumen success .
	manualset3
245531	5	422320	7	NULL	NULL	0	NULL	high patent lumen success	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The contemporary , perineal , one-stage bulboprostatic anastomotic operation as popularized by Turner-Warwick ( 20 ) with selective scar excision is a versatile procedure with a high patent lumen success .
	manualset3
245545	1	422321	7	NULL	NULL	0	NULL	trichogram	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The trichogram also plays a significant role for the diagnosis of the loose anagen hair ( loose anagen syndrome ) , a fairly new , but not rare entity , especially in distinguishing it from telogen effluvium .
	manualset3
245546	2	422321	7	NULL	NULL	0	NULL	 role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The trichogram also plays a significant role for the diagnosis of the loose anagen hair ( loose anagen syndrome ) , a fairly new , but not rare entity , especially in distinguishing it from telogen effluvium .
	manualset3
245547	3	422321	7	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The trichogram also plays a significant role for the diagnosis of the loose anagen hair ( loose anagen syndrome ) , a fairly new , but not rare entity , especially in distinguishing it from telogen effluvium .
	manualset3
245548	4	422321	7	NULL	NULL	0	NULL	loose anagen hair	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	The trichogram also plays a significant role for the diagnosis of the loose anagen hair ( loose anagen syndrome ) , a fairly new , but not rare entity , especially in distinguishing it from telogen effluvium .
	manualset3
245549	5	422321	7	NULL	NULL	0	NULL	loose anagen syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The trichogram also plays a significant role for the diagnosis of the loose anagen hair ( loose anagen syndrome ) , a fairly new , but not rare entity , especially in distinguishing it from telogen effluvium .
	manualset3
245551	6	422321	7	NULL	NULL	0	NULL	rare entity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The trichogram also plays a significant role for the diagnosis of the loose anagen hair ( loose anagen syndrome ) , a fairly new , but not rare entity , especially in distinguishing it from telogen effluvium .
	manualset3
245552	7	422321	7	NULL	NULL	0	NULL	telogen effluvium	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	The trichogram also plays a significant role for the diagnosis of the loose anagen hair ( loose anagen syndrome ) , a fairly new , but not rare entity , especially in distinguishing it from telogen effluvium .
	manualset3
245557	1	422322	7	NULL	NULL	0	NULL	immunosuppressive agent	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	An immunosuppressive agent , FTY720 , increases intracellular concentration of calcium ion and induces apoptosis in HL-60 .
	manualset3
245558	2	422322	7	NULL	NULL	0	NULL	FTY720 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	An immunosuppressive agent , FTY720 , increases intracellular concentration of calcium ion and induces apoptosis in HL-60 .
	manualset3
245559	3	422322	7	NULL	NULL	0	NULL	intracellular concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An immunosuppressive agent , FTY720 , increases intracellular concentration of calcium ion and induces apoptosis in HL-60 .
	manualset3
245561	4	422322	7	NULL	NULL	0	NULL	calcium ion	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	An immunosuppressive agent , FTY720 , increases intracellular concentration of calcium ion and induces apoptosis in HL-60 .
	manualset3
245563	5	422322	7	NULL	NULL	0	NULL	apoptosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	An immunosuppressive agent , FTY720 , increases intracellular concentration of calcium ion and induces apoptosis in HL-60 .
	manualset3
245564	6	422322	7	NULL	NULL	0	NULL	HL-60	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	An immunosuppressive agent , FTY720 , increases intracellular concentration of calcium ion and induces apoptosis in HL-60 .
	manualset3
245565	1	422323	7	NULL	NULL	0	NULL	Excited state dynamics 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Excited state dynamics and rapid internal conversion in a stable dipole molecule .
	manualset3
245566	2	422323	7	NULL	NULL	0	NULL	rapid internal conversion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Excited state dynamics and rapid internal conversion in a stable dipole molecule .
	manualset3
245568	3	422323	7	NULL	NULL	0	NULL	stable dipole molecule	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Excited state dynamics and rapid internal conversion in a stable dipole molecule .
	manualset3
245602	1	422324	7	NULL	NULL	0	NULL	special interest	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Of special interest are women who rely on the traditional method of withdrawal and the proportion of withdrawal failures resulting in abortion .
	manualset3
245603	2	422324	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Of special interest are women who rely on the traditional method of withdrawal and the proportion of withdrawal failures resulting in abortion .
	manualset3
245604	3	422324	7	NULL	NULL	0	NULL	traditional method	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Of special interest are women who rely on the traditional method of withdrawal and the proportion of withdrawal failures resulting in abortion .
	manualset3
245605	4	422324	7	NULL	NULL	0	NULL	withdrawal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Of special interest are women who rely on the traditional method of withdrawal and the proportion of withdrawal failures resulting in abortion .
	manualset3
245607	5	422324	7	NULL	NULL	0	NULL	 proportion	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Of special interest are women who rely on the traditional method of withdrawal and the proportion of withdrawal failures resulting in abortion .
	manualset3
245608	6	422324	7	NULL	NULL	0	NULL	 withdrawal failures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Of special interest are women who rely on the traditional method of withdrawal and the proportion of withdrawal failures resulting in abortion .
	manualset3
245611	7	422324	7	NULL	NULL	0	NULL	abortion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Of special interest are women who rely on the traditional method of withdrawal and the proportion of withdrawal failures resulting in abortion .
	manualset3
245613	1	422325	7	NULL	NULL	0	NULL	Spiny neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Spiny neurons in the neostriatum are highly vulnerable to cerebral ischemia .
	manualset3
245615	2	422325	7	NULL	NULL	0	NULL	neostriatum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Spiny neurons in the neostriatum are highly vulnerable to cerebral ischemia .
	manualset3
245617	3	422325	7	NULL	NULL	0	NULL	cerebral ischemia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Spiny neurons in the neostriatum are highly vulnerable to cerebral ischemia .
	manualset3
245618	1	422326	7	NULL	NULL	0	NULL	 invertebrate system 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In this invertebrate system , glutamate has been identified as the mediator of this signaling in being first released from the active axons thus setting off a series of cascades , leading to a cholinergic activation of the Schwann cell membrane .
	manualset3
245619	2	422326	7	NULL	NULL	0	NULL	glutamate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this invertebrate system , glutamate has been identified as the mediator of this signaling in being first released from the active axons thus setting off a series of cascades , leading to a cholinergic activation of the Schwann cell membrane .
	manualset3
245620	3	422326	7	NULL	NULL	0	NULL	 mediator	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	In this invertebrate system , glutamate has been identified as the mediator of this signaling in being first released from the active axons thus setting off a series of cascades , leading to a cholinergic activation of the Schwann cell membrane .
	manualset3
245622	4	422326	7	NULL	NULL	0	NULL	signaling 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this invertebrate system , glutamate has been identified as the mediator of this signaling in being first released from the active axons thus setting off a series of cascades , leading to a cholinergic activation of the Schwann cell membrane .
	manualset3
245623	5	422326	7	NULL	NULL	0	NULL	active axons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	In this invertebrate system , glutamate has been identified as the mediator of this signaling in being first released from the active axons thus setting off a series of cascades , leading to a cholinergic activation of the Schwann cell membrane .
	manualset3
245624	6	422326	7	NULL	NULL	0	NULL	series	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In this invertebrate system , glutamate has been identified as the mediator of this signaling in being first released from the active axons thus setting off a series of cascades , leading to a cholinergic activation of the Schwann cell membrane .
	manualset3
245626	7	422326	7	NULL	NULL	0	NULL	cascades	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	In this invertebrate system , glutamate has been identified as the mediator of this signaling in being first released from the active axons thus setting off a series of cascades , leading to a cholinergic activation of the Schwann cell membrane .
	manualset3
245628	8	422326	7	NULL	NULL	0	NULL	cholinergic activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In this invertebrate system , glutamate has been identified as the mediator of this signaling in being first released from the active axons thus setting off a series of cascades , leading to a cholinergic activation of the Schwann cell membrane .
	manualset3
245629	9	422326	7	NULL	NULL	0	NULL	Schwann cell membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	In this invertebrate system , glutamate has been identified as the mediator of this signaling in being first released from the active axons thus setting off a series of cascades , leading to a cholinergic activation of the Schwann cell membrane .
	manualset3
245631	1	422327	7	NULL	NULL	0	NULL	Complementation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Complementation of the gene-knock with the full-length gene restored virulence and insect epicuticle germination to wild-type levels .
	manualset3
245633	2	422327	7	NULL	NULL	0	NULL	gene-knock	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Complementation of the gene-knock with the full-length gene restored virulence and insect epicuticle germination to wild-type levels .
	manualset3
245635	3	422327	7	NULL	NULL	0	NULL	full-length gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Complementation of the gene-knock with the full-length gene restored virulence and insect epicuticle germination to wild-type levels .
	manualset3
245637	4	422327	7	NULL	NULL	NULL	NULL	 virulence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Complementation of the gene-knock with the full-length gene restored virulence and insect epicuticle germination to wild-type levels .
	manualset3
245639	5	422327	7	NULL	NULL	0	NULL	insect epicuticle germination	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Complementation of the gene-knock with the full-length gene restored virulence and insect epicuticle germination to wild-type levels .
	manualset3
245640	6	422327	7	NULL	NULL	0	NULL	wild-type levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Complementation of the gene-knock with the full-length gene restored virulence and insect epicuticle germination to wild-type levels .
	manualset3
245642	1	422328	7	NULL	NULL	0	NULL	Synopsis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Synopsis Many of the properties of surfactants can be related to their ability to concentrate at phase interfaces , leading to a reduction in interracial tension .
	manualset3
245643	2	422328	7	NULL	NULL	0	NULL	surfactants	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Synopsis Many of the properties of surfactants can be related to their ability to concentrate at phase interfaces , leading to a reduction in interracial tension .
	manualset3
245645	3	422328	7	NULL	NULL	0	NULL	phase interfaces	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Synopsis Many of the properties of surfactants can be related to their ability to concentrate at phase interfaces , leading to a reduction in interracial tension .
	manualset3
245646	4	422328	7	NULL	NULL	0	NULL	 reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Synopsis Many of the properties of surfactants can be related to their ability to concentrate at phase interfaces , leading to a reduction in interracial tension .
	manualset3
245648	5	422328	7	NULL	NULL	0	NULL	interracial tension	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Synopsis Many of the properties of surfactants can be related to their ability to concentrate at phase interfaces , leading to a reduction in interracial tension .
	manualset3
245650	1	422329	7	NULL	NULL	0	NULL	TPA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although TPA and IL-1 are both potent comitogens for murine thymocytes they markedly differ in their effects on protein phosphorylation and protein kinase C activation .
	manualset3
245651	2	422329	7	NULL	NULL	0	NULL	IL-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although TPA and IL-1 are both potent comitogens for murine thymocytes they markedly differ in their effects on protein phosphorylation and protein kinase C activation .
	manualset3
245652	3	422329	7	NULL	NULL	0	NULL	comitogens	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Although TPA and IL-1 are both potent comitogens for murine thymocytes they markedly differ in their effects on protein phosphorylation and protein kinase C activation .
	manualset3
245653	4	422329	7	NULL	NULL	0	NULL	murine thymocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Although TPA and IL-1 are both potent comitogens for murine thymocytes they markedly differ in their effects on protein phosphorylation and protein kinase C activation .
	manualset3
245654	5	422329	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Although TPA and IL-1 are both potent comitogens for murine thymocytes they markedly differ in their effects on protein phosphorylation and protein kinase C activation .
	manualset3
245655	6	422329	7	NULL	NULL	0	NULL	protein phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although TPA and IL-1 are both potent comitogens for murine thymocytes they markedly differ in their effects on protein phosphorylation and protein kinase C activation .
	manualset3
245656	7	422329	7	NULL	NULL	0	NULL	protein kinase C activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Although TPA and IL-1 are both potent comitogens for murine thymocytes they markedly differ in their effects on protein phosphorylation and protein kinase C activation .
	manualset3
245658	1	422330	7	NULL	NULL	0	NULL	whole cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubating whole cells with the same concentration results in an intranuclear concentration of up to 6 mmol/l after 3 h. The kinetic parameters ( KM = 0.34 mmol/l , Vmax = 0.12 fmol per cell and minute ) are in the same order of magnitude as previously published data .
	manualset3
245660	2	422330	7	NULL	NULL	0	NULL	concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubating whole cells with the same concentration results in an intranuclear concentration of up to 6 mmol/l after 3 h. The kinetic parameters ( KM = 0.34 mmol/l , Vmax = 0.12 fmol per cell and minute ) are in the same order of magnitude as previously published data .
	manualset3
245661	3	422330	7	NULL	NULL	0	NULL	intranuclear concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubating whole cells with the same concentration results in an intranuclear concentration of up to 6 mmol/l after 3 h. The kinetic parameters ( KM = 0.34 mmol/l , Vmax = 0.12 fmol per cell and minute ) are in the same order of magnitude as previously published data .
	manualset3
245662	4	422330	7	NULL	NULL	0	NULL	6 mmol/l	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubating whole cells with the same concentration results in an intranuclear concentration of up to 6 mmol/l after 3 h. The kinetic parameters ( KM = 0.34 mmol/l , Vmax = 0.12 fmol per cell and minute ) are in the same order of magnitude as previously published data .
	manualset3
245663	5	422330	7	NULL	NULL	0	NULL	3 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubating whole cells with the same concentration results in an intranuclear concentration of up to 6 mmol/l after 3 h. The kinetic parameters ( KM = 0.34 mmol/l , Vmax = 0.12 fmol per cell and minute ) are in the same order of magnitude as previously published data .
	manualset3
245665	6	422330	7	NULL	NULL	0	NULL	kinetic parameters	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubating whole cells with the same concentration results in an intranuclear concentration of up to 6 mmol/l after 3 h. The kinetic parameters ( KM = 0.34 mmol/l , Vmax = 0.12 fmol per cell and minute ) are in the same order of magnitude as previously published data .
	manualset3
245667	7	422330	7	NULL	NULL	0	NULL	KM = 0.34 mmol/l 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubating whole cells with the same concentration results in an intranuclear concentration of up to 6 mmol/l after 3 h. The kinetic parameters ( KM = 0.34 mmol/l , Vmax = 0.12 fmol per cell and minute ) are in the same order of magnitude as previously published data .
	manualset3
245669	8	422330	7	NULL	NULL	NULL	NULL	Vmax = 0.12 fmol per cell and minute	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Incubating whole cells with the same concentration results in an intranuclear concentration of up to 6 mmol/l after 3 h. The kinetic parameters ( KM = 0.34 mmol/l , Vmax = 0.12 fmol per cell and minute ) are in the same order of magnitude as previously published data .
	manualset3
245673	9	422330	7	NULL	NULL	0	NULL	 order	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubating whole cells with the same concentration results in an intranuclear concentration of up to 6 mmol/l after 3 h. The kinetic parameters ( KM = 0.34 mmol/l , Vmax = 0.12 fmol per cell and minute ) are in the same order of magnitude as previously published data .
	manualset3
245674	10	422330	7	NULL	NULL	0	NULL	magnitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubating whole cells with the same concentration results in an intranuclear concentration of up to 6 mmol/l after 3 h. The kinetic parameters ( KM = 0.34 mmol/l , Vmax = 0.12 fmol per cell and minute ) are in the same order of magnitude as previously published data .
	manualset3
245675	11	422330	7	NULL	NULL	0	NULL	 published data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Incubating whole cells with the same concentration results in an intranuclear concentration of up to 6 mmol/l after 3 h. The kinetic parameters ( KM = 0.34 mmol/l , Vmax = 0.12 fmol per cell and minute ) are in the same order of magnitude as previously published data .
	manualset3
236611	1	423331	15	NULL	NULL	0	NULL	patella	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Absent patella and contralateral patella alta observed with scoliosis .
	manualset3
236612	2	423331	15	NULL	NULL	0	NULL	contralateral patella alta	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Absent patella and contralateral patella alta observed with scoliosis .
	manualset3
236613	3	423331	15	NULL	NULL	0	NULL	scoliosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Absent patella and contralateral patella alta observed with scoliosis .
	manualset3
236614	1	423332	15	NULL	NULL	0	NULL	Photorhabdus luminescens 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Photorhabdus luminescens is carried in the gut of the infective juvenile ( IJ ) , a nematode stage that infects soft-cuticled insect larvae in the soil .
	manualset3
236615	2	423332	15	NULL	NULL	0	NULL	gut	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Photorhabdus luminescens is carried in the gut of the infective juvenile ( IJ ) , a nematode stage that infects soft-cuticled insect larvae in the soil .
	manualset3
236616	3	423332	15	NULL	NULL	0	NULL	infective juvenile ( IJ )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Photorhabdus luminescens is carried in the gut of the infective juvenile ( IJ ) , a nematode stage that infects soft-cuticled insect larvae in the soil .
	manualset3
236617	4	423332	15	NULL	NULL	0	NULL	nematode stage	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Photorhabdus luminescens is carried in the gut of the infective juvenile ( IJ ) , a nematode stage that infects soft-cuticled insect larvae in the soil .
	manualset3
236618	5	423332	15	NULL	NULL	0	NULL	 insect larvae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Photorhabdus luminescens is carried in the gut of the infective juvenile ( IJ ) , a nematode stage that infects soft-cuticled insect larvae in the soil .
	manualset3
236625	6	423332	15	NULL	NULL	NULL	NULL	soil 	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Photorhabdus luminescens is carried in the gut of the infective juvenile ( IJ ) , a nematode stage that infects soft-cuticled insect larvae in the soil .
	manualset3
236626	1	423333	15	NULL	NULL	0	NULL	Adjunctive H2-blockade	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Adjunctive H2-blockade can help appropriately selected patients with resistant steatorrhoea .
	manualset3
236627	2	423333	15	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Adjunctive H2-blockade can help appropriately selected patients with resistant steatorrhoea .
	manualset3
236628	3	423333	15	NULL	NULL	0	NULL	resistant steatorrhoea	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Adjunctive H2-blockade can help appropriately selected patients with resistant steatorrhoea .
	manualset3
236629	1	423334	15	NULL	NULL	0	NULL	Radioactive precursor incorporation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioactive precursor incorporation into LH was determined by immunoprecipitation , while immunoreactive LH ( iLH ) content was quantified by RIA .
	manualset3
236630	2	423334	15	NULL	NULL	0	NULL	LH	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioactive precursor incorporation into LH was determined by immunoprecipitation , while immunoreactive LH ( iLH ) content was quantified by RIA .
	manualset3
236631	3	423334	15	NULL	NULL	NULL	NULL	immunoprecipitation	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Radioactive precursor incorporation into LH was determined by immunoprecipitation , while immunoreactive LH ( iLH ) content was quantified by RIA .
	manualset3
236632	4	423334	15	NULL	NULL	0	NULL	 immunoreactive LH ( iLH ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioactive precursor incorporation into LH was determined by immunoprecipitation , while immunoreactive LH ( iLH ) content was quantified by RIA .
	manualset3
236633	5	423334	15	NULL	NULL	0	NULL	RIA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Radioactive precursor incorporation into LH was determined by immunoprecipitation , while immunoreactive LH ( iLH ) content was quantified by RIA .
	manualset3
236634	1	423335	15	NULL	NULL	0	NULL	Sr	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Because Sr incorporates into the bone matrix , it was of interest to determine whether SR may affect matrix mineralization in long-term culture .
	manualset3
236635	2	423335	15	NULL	NULL	0	NULL	bone matrix	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Because Sr incorporates into the bone matrix , it was of interest to determine whether SR may affect matrix mineralization in long-term culture .
	manualset3
236636	3	423335	15	NULL	NULL	0	NULL	interest	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Because Sr incorporates into the bone matrix , it was of interest to determine whether SR may affect matrix mineralization in long-term culture .
	manualset3
236637	4	423335	15	NULL	NULL	0	NULL	SR	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Because Sr incorporates into the bone matrix , it was of interest to determine whether SR may affect matrix mineralization in long-term culture .
	manualset3
236638	5	423335	15	NULL	NULL	0	NULL	matrix mineralization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Because Sr incorporates into the bone matrix , it was of interest to determine whether SR may affect matrix mineralization in long-term culture .
	manualset3
236639	6	423335	15	NULL	NULL	0	NULL	long-term culture	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Because Sr incorporates into the bone matrix , it was of interest to determine whether SR may affect matrix mineralization in long-term culture .
	manualset3
236640	1	423336	15	NULL	NULL	0	NULL	Analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the mechanisms involved in growth inhibition revealed that ZR rapidly increased prostaglandin E2 production and in turn cAMP , which inhibited hMF proliferation , did not affect cAMP levels .
	manualset3
236641	2	423336	15	NULL	NULL	0	NULL	mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the mechanisms involved in growth inhibition revealed that ZR rapidly increased prostaglandin E2 production and in turn cAMP , which inhibited hMF proliferation , did not affect cAMP levels .
	manualset3
236642	3	423336	15	NULL	NULL	0	NULL	growth inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the mechanisms involved in growth inhibition revealed that ZR rapidly increased prostaglandin E2 production and in turn cAMP , which inhibited hMF proliferation , did not affect cAMP levels .
	manualset3
236643	4	423336	15	NULL	NULL	0	NULL	ZR	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the mechanisms involved in growth inhibition revealed that ZR rapidly increased prostaglandin E2 production and in turn cAMP , which inhibited hMF proliferation , did not affect cAMP levels .
	manualset3
236644	5	423336	15	NULL	NULL	0	NULL	prostaglandin E2 production	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the mechanisms involved in growth inhibition revealed that ZR rapidly increased prostaglandin E2 production and in turn cAMP , which inhibited hMF proliferation , did not affect cAMP levels .
	manualset3
236645	6	423336	15	NULL	NULL	0	NULL	cAMP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the mechanisms involved in growth inhibition revealed that ZR rapidly increased prostaglandin E2 production and in turn cAMP , which inhibited hMF proliferation , did not affect cAMP levels .
	manualset3
236646	7	423336	15	NULL	NULL	0	NULL	hMF proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the mechanisms involved in growth inhibition revealed that ZR rapidly increased prostaglandin E2 production and in turn cAMP , which inhibited hMF proliferation , did not affect cAMP levels .
	manualset3
236647	8	423336	15	NULL	NULL	0	NULL	cAMP levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the mechanisms involved in growth inhibition revealed that ZR rapidly increased prostaglandin E2 production and in turn cAMP , which inhibited hMF proliferation , did not affect cAMP levels .
	manualset3
236648	1	423337	15	NULL	NULL	0	NULL	asymptomatic activation of the virus	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( i ) Initial , asymptomatic and reversible activation of the virus , judged by the presence of inclusion bearing cells in the urine .
	manualset3
236649	2	423337	15	NULL	NULL	0	NULL	reversible activation of the virus	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( i ) Initial , asymptomatic and reversible activation of the virus , judged by the presence of inclusion bearing cells in the urine .
	manualset3
236650	3	423337	15	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( i ) Initial , asymptomatic and reversible activation of the virus , judged by the presence of inclusion bearing cells in the urine .
	manualset3
236651	4	423337	15	NULL	NULL	0	NULL	inclusion	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	( i ) Initial , asymptomatic and reversible activation of the virus , judged by the presence of inclusion bearing cells in the urine .
	manualset3
236652	5	423337	15	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	( i ) Initial , asymptomatic and reversible activation of the virus , judged by the presence of inclusion bearing cells in the urine .
	manualset3
236653	6	423337	15	NULL	NULL	0	NULL	urine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( i ) Initial , asymptomatic and reversible activation of the virus , judged by the presence of inclusion bearing cells in the urine .
	manualset3
236654	1	423338	15	NULL	NULL	0	NULL	case	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( A case of retinal filariasis ) .
	manualset3
236655	2	423338	15	NULL	NULL	0	NULL	retinal filariasis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( A case of retinal filariasis ) .
	manualset3
236656	1	423339	15	NULL	NULL	0	NULL	Tubulopapillary carcinoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Tubulopapillary carcinoma with spindle cell metaplasia of the mammary gland in a cat .
	manualset3
236657	2	423339	15	NULL	NULL	0	NULL	spindle cell metaplasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Tubulopapillary carcinoma with spindle cell metaplasia of the mammary gland in a cat .
	manualset3
236658	3	423339	15	NULL	NULL	0	NULL	mammary gland	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Tubulopapillary carcinoma with spindle cell metaplasia of the mammary gland in a cat .
	manualset3
236659	4	423339	15	NULL	NULL	0	NULL	cat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Tubulopapillary carcinoma with spindle cell metaplasia of the mammary gland in a cat .
	manualset3
236660	1	423340	15	NULL	NULL	0	NULL	15d-PGJ2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We conclude that 15d-PGJ2 induces endothelial cell apoptosis via a PPAR-dependent pathway .
	manualset3
236661	2	423340	15	NULL	NULL	0	NULL	endothelial cell apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We conclude that 15d-PGJ2 induces endothelial cell apoptosis via a PPAR-dependent pathway .
	manualset3
236662	3	423340	15	NULL	NULL	0	NULL	PPAR-dependent pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We conclude that 15d-PGJ2 induces endothelial cell apoptosis via a PPAR-dependent pathway .
	manualset3
236663	1	423341	15	NULL	NULL	0	NULL	CONCLUSION	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	CONCLUSION : Incidence figures of hospitalization due to RSV infection in this high-risk group of infants were similar to the results from several other reports .
	manualset3
236664	2	423341	15	NULL	NULL	0	NULL	Incidence figures 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	CONCLUSION : Incidence figures of hospitalization due to RSV infection in this high-risk group of infants were similar to the results from several other reports .
	manualset3
236665	3	423341	15	NULL	NULL	0	NULL	hospitalization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	CONCLUSION : Incidence figures of hospitalization due to RSV infection in this high-risk group of infants were similar to the results from several other reports .
	manualset3
236666	4	423341	15	NULL	NULL	0	NULL	RSV infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	CONCLUSION : Incidence figures of hospitalization due to RSV infection in this high-risk group of infants were similar to the results from several other reports .
	manualset3
236667	5	423341	15	NULL	NULL	0	NULL	high-risk group of infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	CONCLUSION : Incidence figures of hospitalization due to RSV infection in this high-risk group of infants were similar to the results from several other reports .
	manualset3
236668	6	423341	15	NULL	NULL	0	NULL	results	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	CONCLUSION : Incidence figures of hospitalization due to RSV infection in this high-risk group of infants were similar to the results from several other reports .
	manualset3
236669	7	423341	15	NULL	NULL	0	NULL	reports	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	CONCLUSION : Incidence figures of hospitalization due to RSV infection in this high-risk group of infants were similar to the results from several other reports .
	manualset3
236670	1	423342	15	NULL	NULL	0	NULL	Electron microscopic observations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Electron microscopic observations on the retino-preoptic pathway of Rana temporaria L .
	manualset3
236671	2	423342	15	NULL	NULL	0	NULL	retino-preoptic pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Electron microscopic observations on the retino-preoptic pathway of Rana temporaria L .
	manualset3
236672	3	423342	15	NULL	NULL	0	NULL	Rana temporaria L	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Electron microscopic observations on the retino-preoptic pathway of Rana temporaria L .
	manualset3
236673	1	423343	15	NULL	NULL	0	NULL	cyclin-dependent kinase inhibitor p27 ( Kip1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	The cyclin-dependent kinase inhibitor p27 ( Kip1 ) is a critical regulator of T cell proliferation .
	manualset3
236674	2	423343	15	NULL	NULL	0	NULL	critical regulator 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The cyclin-dependent kinase inhibitor p27 ( Kip1 ) is a critical regulator of T cell proliferation .
	manualset3
236675	3	423343	15	NULL	NULL	0	NULL	T cell proliferation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cyclin-dependent kinase inhibitor p27 ( Kip1 ) is a critical regulator of T cell proliferation .
	manualset3
236676	1	423344	15	NULL	NULL	0	NULL	Analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the mitochondrial genome contributed towards the elucidation of a number of deviations-deletions or point mutations in mtDNA which are considered the cause of some pathological conditions , usually neuro - and myopathies .
	manualset3
236677	2	423344	15	NULL	NULL	0	NULL	mitochondrial genome	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the mitochondrial genome contributed towards the elucidation of a number of deviations-deletions or point mutations in mtDNA which are considered the cause of some pathological conditions , usually neuro - and myopathies .
	manualset3
236678	3	423344	15	NULL	NULL	0	NULL	elucidation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the mitochondrial genome contributed towards the elucidation of a number of deviations-deletions or point mutations in mtDNA which are considered the cause of some pathological conditions , usually neuro - and myopathies .
	manualset3
236679	4	423344	15	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the mitochondrial genome contributed towards the elucidation of a number of deviations-deletions or point mutations in mtDNA which are considered the cause of some pathological conditions , usually neuro - and myopathies .
	manualset3
236680	5	423344	15	NULL	NULL	0	NULL	deviations-deletions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the mitochondrial genome contributed towards the elucidation of a number of deviations-deletions or point mutations in mtDNA which are considered the cause of some pathological conditions , usually neuro - and myopathies .
	manualset3
236681	6	423344	15	NULL	NULL	0	NULL	point mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the mitochondrial genome contributed towards the elucidation of a number of deviations-deletions or point mutations in mtDNA which are considered the cause of some pathological conditions , usually neuro - and myopathies .
	manualset3
236682	7	423344	15	NULL	NULL	0	NULL	mtDNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the mitochondrial genome contributed towards the elucidation of a number of deviations-deletions or point mutations in mtDNA which are considered the cause of some pathological conditions , usually neuro - and myopathies .
	manualset3
236683	8	423344	15	NULL	NULL	0	NULL	cause 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the mitochondrial genome contributed towards the elucidation of a number of deviations-deletions or point mutations in mtDNA which are considered the cause of some pathological conditions , usually neuro - and myopathies .
	manualset3
236684	9	423344	15	NULL	NULL	0	NULL	pathological conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the mitochondrial genome contributed towards the elucidation of a number of deviations-deletions or point mutations in mtDNA which are considered the cause of some pathological conditions , usually neuro - and myopathies .
	manualset3
236685	10	423344	15	NULL	NULL	0	NULL	neuropathies 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the mitochondrial genome contributed towards the elucidation of a number of deviations-deletions or point mutations in mtDNA which are considered the cause of some pathological conditions , usually neuro - and myopathies .
	manualset3
236686	11	423344	15	NULL	NULL	0	NULL	myopathies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the mitochondrial genome contributed towards the elucidation of a number of deviations-deletions or point mutations in mtDNA which are considered the cause of some pathological conditions , usually neuro - and myopathies .
	manualset3
236687	1	423345	15	NULL	NULL	0	NULL	Value	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Value and limitations of carotid sinus massage in healthy elderly individuals .
	manualset3
236688	2	423345	15	NULL	NULL	0	NULL	limitations 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Value and limitations of carotid sinus massage in healthy elderly individuals .
	manualset3
236689	3	423345	15	NULL	NULL	0	NULL	carotid sinus massage	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Value and limitations of carotid sinus massage in healthy elderly individuals .
	manualset3
236690	4	423345	15	NULL	NULL	0	NULL	healthy elderly individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Value and limitations of carotid sinus massage in healthy elderly individuals .
	manualset3
236691	1	423346	15	NULL	NULL	0	NULL	relationship quality	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	This suggests that while relationship quality determines PC anxiety , it is dependent on the role of the participants in the conflict .
	manualset3
236692	2	423346	15	NULL	NULL	0	NULL	PC anxiety	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This suggests that while relationship quality determines PC anxiety , it is dependent on the role of the participants in the conflict .
	manualset3
236693	3	423346	15	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This suggests that while relationship quality determines PC anxiety , it is dependent on the role of the participants in the conflict .
	manualset3
236694	4	423346	15	NULL	NULL	0	NULL	participants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This suggests that while relationship quality determines PC anxiety , it is dependent on the role of the participants in the conflict .
	manualset3
236695	5	423346	15	NULL	NULL	0	NULL	conflict	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This suggests that while relationship quality determines PC anxiety , it is dependent on the role of the participants in the conflict .
	manualset3
236696	1	423347	15	NULL	NULL	0	NULL	results	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained with this animal model of drug abuse define conditions under which combinations of environmental stimuli might substantially increase human drug use .
	manualset3
236697	2	423347	15	NULL	NULL	0	NULL	animal model of drug abuse	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained with this animal model of drug abuse define conditions under which combinations of environmental stimuli might substantially increase human drug use .
	manualset3
236698	3	423347	15	NULL	NULL	0	NULL	conditions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained with this animal model of drug abuse define conditions under which combinations of environmental stimuli might substantially increase human drug use .
	manualset3
236699	4	423347	15	NULL	NULL	0	NULL	combinations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained with this animal model of drug abuse define conditions under which combinations of environmental stimuli might substantially increase human drug use .
	manualset3
236700	5	423347	15	NULL	NULL	0	NULL	environmental stimuli 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained with this animal model of drug abuse define conditions under which combinations of environmental stimuli might substantially increase human drug use .
	manualset3
236701	6	423347	15	NULL	NULL	0	NULL	human drug use 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The results obtained with this animal model of drug abuse define conditions under which combinations of environmental stimuli might substantially increase human drug use .
	manualset3
236702	1	423348	15	NULL	NULL	0	NULL	thresholds	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These thresholds were determined for three bandwidths of interaurally altered noise ( 2 , 10 , and 100 Hz ) centered at four center frequencies ( 200 , 500 , 1000 , and 1600 Hz ) .
	manualset3
236703	2	423348	15	NULL	NULL	0	NULL	three bandwidths	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These thresholds were determined for three bandwidths of interaurally altered noise ( 2 , 10 , and 100 Hz ) centered at four center frequencies ( 200 , 500 , 1000 , and 1600 Hz ) .
	manualset3
236704	3	423348	15	NULL	NULL	0	NULL	noise 2 Hz	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These thresholds were determined for three bandwidths of interaurally altered noise ( 2 , 10 , and 100 Hz ) centered at four center frequencies ( 200 , 500 , 1000 , and 1600 Hz ) .
	manualset3
236705	4	423348	15	NULL	NULL	0	NULL	noise10 Hz	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These thresholds were determined for three bandwidths of interaurally altered noise ( 2 , 10 , and 100 Hz ) centered at four center frequencies ( 200 , 500 , 1000 , and 1600 Hz ) .
	manualset3
236706	5	423348	15	NULL	NULL	0	NULL	noise 100 Hz	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These thresholds were determined for three bandwidths of interaurally altered noise ( 2 , 10 , and 100 Hz ) centered at four center frequencies ( 200 , 500 , 1000 , and 1600 Hz ) .
	manualset3
236707	6	423348	15	NULL	NULL	0	NULL	four	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	These thresholds were determined for three bandwidths of interaurally altered noise ( 2 , 10 , and 100 Hz ) centered at four center frequencies ( 200 , 500 , 1000 , and 1600 Hz ) .
	manualset3
236708	7	423348	15	NULL	NULL	0	NULL	frequencies 200 Hz	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These thresholds were determined for three bandwidths of interaurally altered noise ( 2 , 10 , and 100 Hz ) centered at four center frequencies ( 200 , 500 , 1000 , and 1600 Hz ) .
	manualset3
236709	8	423348	15	NULL	NULL	0	NULL	frequencies 500 Hz	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These thresholds were determined for three bandwidths of interaurally altered noise ( 2 , 10 , and 100 Hz ) centered at four center frequencies ( 200 , 500 , 1000 , and 1600 Hz ) .
	manualset3
236710	9	423348	15	NULL	NULL	0	NULL	frequencies 1000 Hz	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These thresholds were determined for three bandwidths of interaurally altered noise ( 2 , 10 , and 100 Hz ) centered at four center frequencies ( 200 , 500 , 1000 , and 1600 Hz ) .
	manualset3
236711	10	423348	15	NULL	NULL	0	NULL	frequencies 1600 Hz	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	These thresholds were determined for three bandwidths of interaurally altered noise ( 2 , 10 , and 100 Hz ) centered at four center frequencies ( 200 , 500 , 1000 , and 1600 Hz ) .
	manualset3
236712	1	423349	15	NULL	NULL	0	NULL	cAMP blockers H89 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , cAMP blockers H89 and Rp-cAMP failed to block the effect of PGD2 .
	manualset3
236713	2	423349	15	NULL	NULL	0	NULL	cAMP blockers Rp-cAMP	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	However , cAMP blockers H89 and Rp-cAMP failed to block the effect of PGD2 .
	manualset3
236714	3	423349	15	NULL	NULL	0	NULL	block	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	However , cAMP blockers H89 and Rp-cAMP failed to block the effect of PGD2 .
	manualset3
236715	4	423349	15	NULL	NULL	0	NULL	effect of PGD2	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	However , cAMP blockers H89 and Rp-cAMP failed to block the effect of PGD2 .
	manualset3
236716	1	423350	15	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	It follows that analysis of melanocytes cultured from vitiligo donors can contribute to a further understanding of the etiopathomechanism .
	manualset3
236717	2	423350	15	NULL	NULL	0	NULL	melanocytes 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	It follows that analysis of melanocytes cultured from vitiligo donors can contribute to a further understanding of the etiopathomechanism .
	manualset3
236718	3	423350	15	NULL	NULL	0	NULL	vitiligo donors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	It follows that analysis of melanocytes cultured from vitiligo donors can contribute to a further understanding of the etiopathomechanism .
	manualset3
236719	4	423350	15	NULL	NULL	0	NULL	understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It follows that analysis of melanocytes cultured from vitiligo donors can contribute to a further understanding of the etiopathomechanism .
	manualset3
236720	5	423350	15	NULL	NULL	0	NULL	etiopathomechanism 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It follows that analysis of melanocytes cultured from vitiligo donors can contribute to a further understanding of the etiopathomechanism .
	manualset3
236721	1	423351	15	NULL	NULL	0	NULL	Susceptibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Susceptibility to foot-and-mouth disease virus ) .
	manualset3
236722	2	423351	15	NULL	NULL	0	NULL	 foot-and-mouth disease virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Susceptibility to foot-and-mouth disease virus ) .
	manualset3
236723	1	423352	15	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	From these studies we conclude that putative promoter sequences in M. hyopneumoniae deviate significantly from those in Escherichia coli and Bacillus subtilis in having its -35 consensus sequence replaced by A-T rich sequences , whereas the characterized M. capricolum promoter resembles more closely a typical E. coli promoter .
	manualset3
236724	2	423352	15	NULL	NULL	0	NULL	putative promoter sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	From these studies we conclude that putative promoter sequences in M. hyopneumoniae deviate significantly from those in Escherichia coli and Bacillus subtilis in having its -35 consensus sequence replaced by A-T rich sequences , whereas the characterized M. capricolum promoter resembles more closely a typical E. coli promoter .
	manualset3
236725	3	423352	15	NULL	NULL	0	NULL	M. hyopneumoniae 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	From these studies we conclude that putative promoter sequences in M. hyopneumoniae deviate significantly from those in Escherichia coli and Bacillus subtilis in having its -35 consensus sequence replaced by A-T rich sequences , whereas the characterized M. capricolum promoter resembles more closely a typical E. coli promoter .
	manualset3
236726	4	423352	15	NULL	NULL	0	NULL	Escherichia coli	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	From these studies we conclude that putative promoter sequences in M. hyopneumoniae deviate significantly from those in Escherichia coli and Bacillus subtilis in having its -35 consensus sequence replaced by A-T rich sequences , whereas the characterized M. capricolum promoter resembles more closely a typical E. coli promoter .
	manualset3
236727	5	423352	15	NULL	NULL	0	NULL	Bacillus subtilis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	From these studies we conclude that putative promoter sequences in M. hyopneumoniae deviate significantly from those in Escherichia coli and Bacillus subtilis in having its -35 consensus sequence replaced by A-T rich sequences , whereas the characterized M. capricolum promoter resembles more closely a typical E. coli promoter .
	manualset3
236728	6	423352	15	NULL	NULL	0	NULL	-35 consensus sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	From these studies we conclude that putative promoter sequences in M. hyopneumoniae deviate significantly from those in Escherichia coli and Bacillus subtilis in having its -35 consensus sequence replaced by A-T rich sequences , whereas the characterized M. capricolum promoter resembles more closely a typical E. coli promoter .
	manualset3
236729	7	423352	15	NULL	NULL	0	NULL	A-T rich sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	From these studies we conclude that putative promoter sequences in M. hyopneumoniae deviate significantly from those in Escherichia coli and Bacillus subtilis in having its -35 consensus sequence replaced by A-T rich sequences , whereas the characterized M. capricolum promoter resembles more closely a typical E. coli promoter .
	manualset3
236730	8	423352	15	NULL	NULL	0	NULL	M. capricolum promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	From these studies we conclude that putative promoter sequences in M. hyopneumoniae deviate significantly from those in Escherichia coli and Bacillus subtilis in having its -35 consensus sequence replaced by A-T rich sequences , whereas the characterized M. capricolum promoter resembles more closely a typical E. coli promoter .
	manualset3
236731	9	423352	15	NULL	NULL	0	NULL	E. coli promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	From these studies we conclude that putative promoter sequences in M. hyopneumoniae deviate significantly from those in Escherichia coli and Bacillus subtilis in having its -35 consensus sequence replaced by A-T rich sequences , whereas the characterized M. capricolum promoter resembles more closely a typical E. coli promoter .
	manualset3
236732	1	423353	15	NULL	NULL	0	NULL	9-kilobase EcoRI fragment	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A 9-kilobase EcoRI fragment containing treA was subcloned into pBR322 .
	manualset3
236733	2	423353	15	NULL	NULL	0	NULL	treA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	A 9-kilobase EcoRI fragment containing treA was subcloned into pBR322 .
	manualset3
236734	3	423353	15	NULL	NULL	0	NULL	pBR322	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	A 9-kilobase EcoRI fragment containing treA was subcloned into pBR322 .
	manualset3
236735	1	423354	15	NULL	NULL	0	NULL	Analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the pleural effusion revealed an increased CD4/CD8 ratio because of an increased percentage of CD4 + CD29 + helper memory T cells , lack of expression of the resting B-cell marker CD21 , immune complex deposition and complement consumption , increased relative levels of ANA , abnormally high levels of IL-6 and soluble IL-2R , and detectable levels of IL-1b , IFN-g and TNF-a .
	manualset3
236736	2	423354	15	NULL	NULL	0	NULL	pleural effusion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the pleural effusion revealed an increased CD4/CD8 ratio because of an increased percentage of CD4 + CD29 + helper memory T cells , lack of expression of the resting B-cell marker CD21 , immune complex deposition and complement consumption , increased relative levels of ANA , abnormally high levels of IL-6 and soluble IL-2R , and detectable levels of IL-1b , IFN-g and TNF-a .
	manualset3
236737	3	423354	15	NULL	NULL	NULL	NULL	CD4/CD8 ratio	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Analysis of the pleural effusion revealed an increased CD4/CD8 ratio because of an increased percentage of CD4 + CD29 + helper memory T cells , lack of expression of the resting B-cell marker CD21 , immune complex deposition and complement consumption , increased relative levels of ANA , abnormally high levels of IL-6 and soluble IL-2R , and detectable levels of IL-1b , IFN-g and TNF-a .
	manualset3
236738	4	423354	15	NULL	NULL	0	NULL	percentage of CD4 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the pleural effusion revealed an increased CD4/CD8 ratio because of an increased percentage of CD4 + CD29 + helper memory T cells , lack of expression of the resting B-cell marker CD21 , immune complex deposition and complement consumption , increased relative levels of ANA , abnormally high levels of IL-6 and soluble IL-2R , and detectable levels of IL-1b , IFN-g and TNF-a .
	manualset3
236739	5	423354	15	NULL	NULL	0	NULL	percentage of CD29	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the pleural effusion revealed an increased CD4/CD8 ratio because of an increased percentage of CD4 + CD29 + helper memory T cells , lack of expression of the resting B-cell marker CD21 , immune complex deposition and complement consumption , increased relative levels of ANA , abnormally high levels of IL-6 and soluble IL-2R , and detectable levels of IL-1b , IFN-g and TNF-a .
	manualset3
236740	6	423354	15	NULL	NULL	0	NULL	percentage of helper memory T cells 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the pleural effusion revealed an increased CD4/CD8 ratio because of an increased percentage of CD4 + CD29 + helper memory T cells , lack of expression of the resting B-cell marker CD21 , immune complex deposition and complement consumption , increased relative levels of ANA , abnormally high levels of IL-6 and soluble IL-2R , and detectable levels of IL-1b , IFN-g and TNF-a .
	manualset3
236741	7	423354	15	NULL	NULL	0	NULL	lack of expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the pleural effusion revealed an increased CD4/CD8 ratio because of an increased percentage of CD4 + CD29 + helper memory T cells , lack of expression of the resting B-cell marker CD21 , immune complex deposition and complement consumption , increased relative levels of ANA , abnormally high levels of IL-6 and soluble IL-2R , and detectable levels of IL-1b , IFN-g and TNF-a .
	manualset3
236836	8	423354	15	NULL	NULL	0	NULL	B-cell marker CD21	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the pleural effusion revealed an increased CD4/CD8 ratio because of an increased percentage of CD4 + CD29 + helper memory T cells , lack of expression of the resting B-cell marker CD21 , immune complex deposition and complement consumption , increased relative levels of ANA , abnormally high levels of IL-6 and soluble IL-2R , and detectable levels of IL-1b , IFN-g and TNF-a .
	manualset3
236837	9	423354	15	NULL	NULL	NULL	NULL	immune complex deposition	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Analysis of the pleural effusion revealed an increased CD4/CD8 ratio because of an increased percentage of CD4 + CD29 + helper memory T cells , lack of expression of the resting B-cell marker CD21 , immune complex deposition and complement consumption , increased relative levels of ANA , abnormally high levels of IL-6 and soluble IL-2R , and detectable levels of IL-1b , IFN-g and TNF-a .
	manualset3
236839	10	423354	15	NULL	NULL	NULL	NULL	complement consumption	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Analysis of the pleural effusion revealed an increased CD4/CD8 ratio because of an increased percentage of CD4 + CD29 + helper memory T cells , lack of expression of the resting B-cell marker CD21 , immune complex deposition and complement consumption , increased relative levels of ANA , abnormally high levels of IL-6 and soluble IL-2R , and detectable levels of IL-1b , IFN-g and TNF-a .
	manualset3
236840	11	423354	15	NULL	NULL	0	NULL	relative levels of ANA	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the pleural effusion revealed an increased CD4/CD8 ratio because of an increased percentage of CD4 + CD29 + helper memory T cells , lack of expression of the resting B-cell marker CD21 , immune complex deposition and complement consumption , increased relative levels of ANA , abnormally high levels of IL-6 and soluble IL-2R , and detectable levels of IL-1b , IFN-g and TNF-a .
	manualset3
236841	12	423354	15	NULL	NULL	0	NULL	high levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the pleural effusion revealed an increased CD4/CD8 ratio because of an increased percentage of CD4 + CD29 + helper memory T cells , lack of expression of the resting B-cell marker CD21 , immune complex deposition and complement consumption , increased relative levels of ANA , abnormally high levels of IL-6 and soluble IL-2R , and detectable levels of IL-1b , IFN-g and TNF-a .
	manualset3
236843	13	423354	15	NULL	NULL	0	NULL	IL-6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the pleural effusion revealed an increased CD4/CD8 ratio because of an increased percentage of CD4 + CD29 + helper memory T cells , lack of expression of the resting B-cell marker CD21 , immune complex deposition and complement consumption , increased relative levels of ANA , abnormally high levels of IL-6 and soluble IL-2R , and detectable levels of IL-1b , IFN-g and TNF-a .
	manualset3
236844	14	423354	15	NULL	NULL	0	NULL	soluble IL-2R	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the pleural effusion revealed an increased CD4/CD8 ratio because of an increased percentage of CD4 + CD29 + helper memory T cells , lack of expression of the resting B-cell marker CD21 , immune complex deposition and complement consumption , increased relative levels of ANA , abnormally high levels of IL-6 and soluble IL-2R , and detectable levels of IL-1b , IFN-g and TNF-a .
	manualset3
236848	15	423354	15	NULL	NULL	0	NULL	detectable levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the pleural effusion revealed an increased CD4/CD8 ratio because of an increased percentage of CD4 + CD29 + helper memory T cells , lack of expression of the resting B-cell marker CD21 , immune complex deposition and complement consumption , increased relative levels of ANA , abnormally high levels of IL-6 and soluble IL-2R , and detectable levels of IL-1b , IFN-g and TNF-a .
	manualset3
236850	16	423354	15	NULL	NULL	0	NULL	IL-1b	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the pleural effusion revealed an increased CD4/CD8 ratio because of an increased percentage of CD4 + CD29 + helper memory T cells , lack of expression of the resting B-cell marker CD21 , immune complex deposition and complement consumption , increased relative levels of ANA , abnormally high levels of IL-6 and soluble IL-2R , and detectable levels of IL-1b , IFN-g and TNF-a .
	manualset3
236851	17	423354	15	NULL	NULL	0	NULL	IFN-g	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the pleural effusion revealed an increased CD4/CD8 ratio because of an increased percentage of CD4 + CD29 + helper memory T cells , lack of expression of the resting B-cell marker CD21 , immune complex deposition and complement consumption , increased relative levels of ANA , abnormally high levels of IL-6 and soluble IL-2R , and detectable levels of IL-1b , IFN-g and TNF-a .
	manualset3
236852	18	423354	15	NULL	NULL	0	NULL	TNF-a	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the pleural effusion revealed an increased CD4/CD8 ratio because of an increased percentage of CD4 + CD29 + helper memory T cells , lack of expression of the resting B-cell marker CD21 , immune complex deposition and complement consumption , increased relative levels of ANA , abnormally high levels of IL-6 and soluble IL-2R , and detectable levels of IL-1b , IFN-g and TNF-a .
	manualset3
236742	1	423355	15	NULL	NULL	0	NULL	record linkage	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Anonymised record linkage of cohort study data with national registry data indicated that selective non-response was present in the ABCD-study , but selection bias was acceptably low and did not influence the main study questions .
	manualset3
236743	2	423355	15	NULL	NULL	NULL	NULL	cohort study data 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Anonymised record linkage of cohort study data with national registry data indicated that selective non-response was present in the ABCD-study , but selection bias was acceptably low and did not influence the main study questions .
	manualset3
236744	3	423355	15	NULL	NULL	NULL	NULL	national registry data 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Anonymised record linkage of cohort study data with national registry data indicated that selective non-response was present in the ABCD-study , but selection bias was acceptably low and did not influence the main study questions .
	manualset3
236745	4	423355	15	NULL	NULL	0	NULL	non-response	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Anonymised record linkage of cohort study data with national registry data indicated that selective non-response was present in the ABCD-study , but selection bias was acceptably low and did not influence the main study questions .
	manualset3
236746	5	423355	15	NULL	NULL	0	NULL	ABCD-study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Anonymised record linkage of cohort study data with national registry data indicated that selective non-response was present in the ABCD-study , but selection bias was acceptably low and did not influence the main study questions .
	manualset3
236750	6	423355	15	NULL	NULL	0	NULL	selection bias	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Anonymised record linkage of cohort study data with national registry data indicated that selective non-response was present in the ABCD-study , but selection bias was acceptably low and did not influence the main study questions .
	manualset3
236754	7	423355	15	NULL	NULL	0	NULL	influence	process												NULL		0	NULL	NULL	NULL	NULL	NULL	Anonymised record linkage of cohort study data with national registry data indicated that selective non-response was present in the ABCD-study , but selection bias was acceptably low and did not influence the main study questions .
	manualset3
236756	8	423355	15	NULL	NULL	0	NULL	study questions	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Anonymised record linkage of cohort study data with national registry data indicated that selective non-response was present in the ABCD-study , but selection bias was acceptably low and did not influence the main study questions .
	manualset3
236747	1	423356	15	NULL	NULL	0	NULL	Pig kidneys	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Pig and human kidneys are anatomically similar ( characterized by multilobular structure in contrast to rodent and dog kidneys unilobular ) .
	manualset3
236748	2	423356	15	NULL	NULL	0	NULL	human kidneys	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Pig and human kidneys are anatomically similar ( characterized by multilobular structure in contrast to rodent and dog kidneys unilobular ) .
	manualset3
236765	3	423356	15	NULL	NULL	0	NULL	multilobular structure	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pig and human kidneys are anatomically similar ( characterized by multilobular structure in contrast to rodent and dog kidneys unilobular ) .
	manualset3
236766	4	423356	15	NULL	NULL	NULL	NULL	contrast	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pig and human kidneys are anatomically similar ( characterized by multilobular structure in contrast to rodent and dog kidneys unilobular ) .
	manualset3
236767	5	423356	15	NULL	NULL	0	NULL	rodent kidneys	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Pig and human kidneys are anatomically similar ( characterized by multilobular structure in contrast to rodent and dog kidneys unilobular ) .
	manualset3
236768	6	423356	15	NULL	NULL	0	NULL	dog kidneys	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Pig and human kidneys are anatomically similar ( characterized by multilobular structure in contrast to rodent and dog kidneys unilobular ) .
	manualset3
236769	7	423356	15	NULL	NULL	0	NULL	unilobular	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pig and human kidneys are anatomically similar ( characterized by multilobular structure in contrast to rodent and dog kidneys unilobular ) .
	manualset3
236772	4	423357	15	NULL	NULL	NULL	NULL	Fijian kawa ( Piper methysticum )	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Isolation and synthesis of TNF-alpha release inhibitors from Fijian kawa ( Piper methysticum ) .
	manualset3
239063	1	423357	15	NULL	NULL	0	NULL	Isolation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation and synthesis of TNF-alpha release inhibitors from Fijian kawa ( Piper methysticum ) .
	manualset3
239064	2	423357	15	NULL	NULL	0	NULL	synthesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation and synthesis of TNF-alpha release inhibitors from Fijian kawa ( Piper methysticum ) .
	manualset3
239065	3	423357	15	NULL	NULL	0	NULL	TNF-alpha release inhibitors	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Isolation and synthesis of TNF-alpha release inhibitors from Fijian kawa ( Piper methysticum ) .
	manualset3
236773	1	423358	15	NULL	NULL	0	NULL	Aneuploidy	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Aneuploidy reduces fecundity and is a frequent cause of inherited birth defects .
	manualset3
236774	2	423358	15	NULL	NULL	0	NULL	fecundity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Aneuploidy reduces fecundity and is a frequent cause of inherited birth defects .
	manualset3
236775	3	423358	15	NULL	NULL	0	NULL	cause	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Aneuploidy reduces fecundity and is a frequent cause of inherited birth defects .
	manualset3
236776	4	423358	15	NULL	NULL	0	NULL	inherited birth defects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Aneuploidy reduces fecundity and is a frequent cause of inherited birth defects .
	manualset3
236777	1	423359	15	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of a prophylactic bolus of lidocaine in focal cerebral ischemia .
	manualset3
236781	2	423359	15	NULL	NULL	0	NULL	prophylactic bolus of lidocaine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of a prophylactic bolus of lidocaine in focal cerebral ischemia .
	manualset3
236783	3	423359	15	NULL	NULL	0	NULL	focal cerebral ischemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The effects of a prophylactic bolus of lidocaine in focal cerebral ischemia .
	manualset3
236790	1	423360	15	NULL	NULL	0	NULL	KA values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The KA values for cAMP were 9.1 and greater than 20 microM for the I alpha and I beta isozymes , respectively .
	manualset3
236792	2	423360	15	NULL	NULL	0	NULL	cAMP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	The KA values for cAMP were 9.1 and greater than 20 microM for the I alpha and I beta isozymes , respectively .
	manualset3
236794	3	423360	15	NULL	NULL	0	NULL	9.1	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The KA values for cAMP were 9.1 and greater than 20 microM for the I alpha and I beta isozymes , respectively .
	manualset3
236796	4	423360	15	NULL	NULL	0	NULL	20 microM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The KA values for cAMP were 9.1 and greater than 20 microM for the I alpha and I beta isozymes , respectively .
	manualset3
236797	5	423360	15	NULL	NULL	0	NULL	I alpha isozymes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The KA values for cAMP were 9.1 and greater than 20 microM for the I alpha and I beta isozymes , respectively .
	manualset3
236798	6	423360	15	NULL	NULL	0	NULL	I beta isozymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The KA values for cAMP were 9.1 and greater than 20 microM for the I alpha and I beta isozymes , respectively .
	manualset3
236801	1	423361	15	NULL	NULL	0	NULL	Analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the promoter region of the acetate-induced isocitrate lyase gene ( acuD ) of Aspergillus nidulans is described .
	manualset3
236802	2	423361	15	NULL	NULL	0	NULL	promoter region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the promoter region of the acetate-induced isocitrate lyase gene ( acuD ) of Aspergillus nidulans is described .
	manualset3
236806	3	423361	15	NULL	NULL	0	NULL	acetate-induced isocitrate lyase gene ( acuD )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the promoter region of the acetate-induced isocitrate lyase gene ( acuD ) of Aspergillus nidulans is described .
	manualset3
236807	4	423361	15	NULL	NULL	0	NULL	Aspergillus nidulans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the promoter region of the acetate-induced isocitrate lyase gene ( acuD ) of Aspergillus nidulans is described .
	manualset3
236810	1	423362	15	NULL	NULL	0	NULL	Associations 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Associations among awareness of prognosis , hopefulness , and coping in patients with advanced cancer participating in phase I clinical trials .
	manualset3
236811	2	423362	15	NULL	NULL	0	NULL	awareness of prognosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Associations among awareness of prognosis , hopefulness , and coping in patients with advanced cancer participating in phase I clinical trials .
	manualset3
236812	3	423362	15	NULL	NULL	0	NULL	hopefulness	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Associations among awareness of prognosis , hopefulness , and coping in patients with advanced cancer participating in phase I clinical trials .
	manualset3
236813	4	423362	15	NULL	NULL	0	NULL	coping in patients	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Associations among awareness of prognosis , hopefulness , and coping in patients with advanced cancer participating in phase I clinical trials .
	manualset3
236814	5	423362	15	NULL	NULL	0	NULL	cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Associations among awareness of prognosis , hopefulness , and coping in patients with advanced cancer participating in phase I clinical trials .
	manualset3
236817	6	423362	15	NULL	NULL	0	NULL	phase I clinical trials	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Associations among awareness of prognosis , hopefulness , and coping in patients with advanced cancer participating in phase I clinical trials .
	manualset3
236818	1	423363	15	NULL	NULL	0	NULL	Hypoxia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypoxia decreased the specific membrane resistance ( Rm ) , but the changes were not statistically significant .
	manualset3
236821	2	423363	15	NULL	NULL	0	NULL	specific membrane resistance ( Rm )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypoxia decreased the specific membrane resistance ( Rm ) , but the changes were not statistically significant .
	manualset3
236825	3	423363	15	NULL	NULL	0	NULL	changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Hypoxia decreased the specific membrane resistance ( Rm ) , but the changes were not statistically significant .
	manualset3
236827	1	423364	15	NULL	NULL	0	NULL	Studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on the control of the corpus luteum in the vole , Microtus agrestis .
	manualset3
236829	2	423364	15	NULL	NULL	0	NULL	control of the corpus luteum	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on the control of the corpus luteum in the vole , Microtus agrestis .
	manualset3
236831	3	423364	15	NULL	NULL	0	NULL	vole , Microtus agrestis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Studies on the control of the corpus luteum in the vole , Microtus agrestis .
	manualset3
236854	1	423365	15	NULL	NULL	0	NULL	Analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the received data showed that in the majority of cases it was expedient to recommend 3 bearing ( abutments ) system of denture making .
	manualset3
236855	2	423365	15	NULL	NULL	NULL	NULL	received data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Analysis of the received data showed that in the majority of cases it was expedient to recommend 3 bearing ( abutments ) system of denture making .
	manualset3
236856	3	423365	15	NULL	NULL	0	NULL	majority of cases	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the received data showed that in the majority of cases it was expedient to recommend 3 bearing ( abutments ) system of denture making .
	manualset3
236857	4	423365	15	NULL	NULL	0	NULL	3 bearing ( abutments ) system of denture making 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the received data showed that in the majority of cases it was expedient to recommend 3 bearing ( abutments ) system of denture making .
	manualset3
236858	1	423366	15	NULL	NULL	0	NULL	etanercept	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	We propose that etanercept may be a suitable drug for patients with RA who desire to become pregnant .
	manualset3
236859	2	423366	15	NULL	NULL	0	NULL	drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	We propose that etanercept may be a suitable drug for patients with RA who desire to become pregnant .
	manualset3
236860	3	423366	15	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	We propose that etanercept may be a suitable drug for patients with RA who desire to become pregnant .
	manualset3
236861	4	423366	15	NULL	NULL	0	NULL	RA	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We propose that etanercept may be a suitable drug for patients with RA who desire to become pregnant .
	manualset3
236862	5	423366	15	NULL	NULL	0	NULL	desire	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We propose that etanercept may be a suitable drug for patients with RA who desire to become pregnant .
	manualset3
236863	6	423366	15	NULL	NULL	0	NULL	pregnant	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We propose that etanercept may be a suitable drug for patients with RA who desire to become pregnant .
	manualset3
236864	1	423367	15	NULL	NULL	0	NULL	Survival 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Survival of a bioaugmented strain , conjugative plasmid transfer and enhanced BA degradation was demonstrated in the laboratory scale SBBR but not in the pilot scale SBBR .
	manualset3
236865	2	423367	15	NULL	NULL	0	NULL	bioaugmented strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Survival of a bioaugmented strain , conjugative plasmid transfer and enhanced BA degradation was demonstrated in the laboratory scale SBBR but not in the pilot scale SBBR .
	manualset3
236866	3	423367	15	NULL	NULL	0	NULL	conjugative plasmid transfer	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Survival of a bioaugmented strain , conjugative plasmid transfer and enhanced BA degradation was demonstrated in the laboratory scale SBBR but not in the pilot scale SBBR .
	manualset3
236867	4	423367	15	NULL	NULL	0	NULL	enhanced BA degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Survival of a bioaugmented strain , conjugative plasmid transfer and enhanced BA degradation was demonstrated in the laboratory scale SBBR but not in the pilot scale SBBR .
	manualset3
236868	5	423367	15	NULL	NULL	0	NULL	laboratory scale SBBR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Survival of a bioaugmented strain , conjugative plasmid transfer and enhanced BA degradation was demonstrated in the laboratory scale SBBR but not in the pilot scale SBBR .
	manualset3
236869	6	423367	15	NULL	NULL	NULL	NULL	pilot scale SBBR	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Survival of a bioaugmented strain , conjugative plasmid transfer and enhanced BA degradation was demonstrated in the laboratory scale SBBR but not in the pilot scale SBBR .
	manualset3
236870	1	423368	15	NULL	NULL	0	NULL	10 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	At least 10 % of people aged 65 or older have some form of cognitive impairment , increasing to around 50 % by age 85 .
	manualset3
236871	2	423368	15	NULL	NULL	0	NULL	people 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	At least 10 % of people aged 65 or older have some form of cognitive impairment , increasing to around 50 % by age 85 .
	manualset3
237135	3	423368	15	NULL	NULL	0	NULL	aged 65	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	At least 10 % of people aged 65 or older have some form of cognitive impairment , increasing to around 50 % by age 85 .
	manualset3
237137	4	423368	15	NULL	NULL	0	NULL	cognitive impairment	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	At least 10 % of people aged 65 or older have some form of cognitive impairment , increasing to around 50 % by age 85 .
	manualset3
237138	5	423368	15	NULL	NULL	0	NULL	50 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	At least 10 % of people aged 65 or older have some form of cognitive impairment , increasing to around 50 % by age 85 .
	manualset3
237140	6	423368	15	NULL	NULL	0	NULL	age 85	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	At least 10 % of people aged 65 or older have some form of cognitive impairment , increasing to around 50 % by age 85 .
	manualset3
236872	1	423369	15	NULL	NULL	0	NULL	Deletion of cymR 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Deletion of cymR reduced the resistance of S. aureus to oxidative stresses , and the resistance was restored by expressing a C25S mutant copy of cymR .
	manualset3
236873	2	423369	15	NULL	NULL	0	NULL	resistance 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Deletion of cymR reduced the resistance of S. aureus to oxidative stresses , and the resistance was restored by expressing a C25S mutant copy of cymR .
	manualset3
236876	3	423369	15	NULL	NULL	0	NULL	S. aureus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Deletion of cymR reduced the resistance of S. aureus to oxidative stresses , and the resistance was restored by expressing a C25S mutant copy of cymR .
	manualset3
236878	4	423369	15	NULL	NULL	0	NULL	oxidative stresses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Deletion of cymR reduced the resistance of S. aureus to oxidative stresses , and the resistance was restored by expressing a C25S mutant copy of cymR .
	manualset3
236880	5	423369	15	NULL	NULL	0	NULL	resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Deletion of cymR reduced the resistance of S. aureus to oxidative stresses , and the resistance was restored by expressing a C25S mutant copy of cymR .
	manualset3
236881	6	423369	15	NULL	NULL	0	NULL	expressing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Deletion of cymR reduced the resistance of S. aureus to oxidative stresses , and the resistance was restored by expressing a C25S mutant copy of cymR .
	manualset3
236887	7	423369	15	NULL	NULL	0	NULL	C25S mutant copy of cymR	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Deletion of cymR reduced the resistance of S. aureus to oxidative stresses , and the resistance was restored by expressing a C25S mutant copy of cymR .
	manualset3
236898	1	423370	15	NULL	NULL	NULL	NULL	models	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We developed models to take into account the complex behavior of airflow patterns in multifamily buildings , which can be used to identify and evaluate environmental and non-environmental interventions targeting indoor air pollutants which can trigger asthma exacerbations .
	manualset3
236902	2	423370	15	NULL	NULL	NULL	NULL	complex behavior 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We developed models to take into account the complex behavior of airflow patterns in multifamily buildings , which can be used to identify and evaluate environmental and non-environmental interventions targeting indoor air pollutants which can trigger asthma exacerbations .
	manualset3
236904	3	423370	15	NULL	NULL	NULL	NULL	airflow patterns	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We developed models to take into account the complex behavior of airflow patterns in multifamily buildings , which can be used to identify and evaluate environmental and non-environmental interventions targeting indoor air pollutants which can trigger asthma exacerbations .
	manualset3
236906	4	423370	15	NULL	NULL	NULL	NULL	multifamily buildings	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We developed models to take into account the complex behavior of airflow patterns in multifamily buildings , which can be used to identify and evaluate environmental and non-environmental interventions targeting indoor air pollutants which can trigger asthma exacerbations .
	manualset3
236909	5	423370	15	NULL	NULL	NULL	NULL	environmental interventions	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We developed models to take into account the complex behavior of airflow patterns in multifamily buildings , which can be used to identify and evaluate environmental and non-environmental interventions targeting indoor air pollutants which can trigger asthma exacerbations .
	manualset3
236911	6	423370	15	NULL	NULL	NULL	NULL	non-environmental interventions	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We developed models to take into account the complex behavior of airflow patterns in multifamily buildings , which can be used to identify and evaluate environmental and non-environmental interventions targeting indoor air pollutants which can trigger asthma exacerbations .
	manualset3
236913	7	423370	15	NULL	NULL	NULL	NULL	indoor air pollutants	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We developed models to take into account the complex behavior of airflow patterns in multifamily buildings , which can be used to identify and evaluate environmental and non-environmental interventions targeting indoor air pollutants which can trigger asthma exacerbations .
	manualset3
236914	8	423370	15	NULL	NULL	NULL	NULL	asthma exacerbations	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	We developed models to take into account the complex behavior of airflow patterns in multifamily buildings , which can be used to identify and evaluate environmental and non-environmental interventions targeting indoor air pollutants which can trigger asthma exacerbations .
	manualset3
236926	1	423371	15	NULL	NULL	NULL	NULL	optical detection 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Combined optical and acoustical detection of single microbubble dynamics .
	manualset3
236927	2	423371	15	NULL	NULL	NULL	NULL	acoustical detection	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Combined optical and acoustical detection of single microbubble dynamics .
	manualset3
236933	3	423371	15	NULL	NULL	0	NULL	single microbubble dynamics	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Combined optical and acoustical detection of single microbubble dynamics .
	manualset3
236935	1	423372	15	NULL	NULL	0	NULL	Short term	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Short term aerobic training improved fitness , but did not increase the GH response to exercise .
	manualset3
236937	2	423372	15	NULL	NULL	0	NULL	aerobic training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Short term aerobic training improved fitness , but did not increase the GH response to exercise .
	manualset3
236939	3	423372	15	NULL	NULL	0	NULL	fitness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Short term aerobic training improved fitness , but did not increase the GH response to exercise .
	manualset3
236940	4	423372	15	NULL	NULL	NULL	NULL	GH response to exercise	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Short term aerobic training improved fitness , but did not increase the GH response to exercise .
	manualset3
236948	1	423373	15	NULL	NULL	0	NULL	Epidemiological considerations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Epidemiological considerations of the problem of suicide ( condition in the Splitz region ) ) .
	manualset3
236949	2	423373	15	NULL	NULL	0	NULL	problem of suicide	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Epidemiological considerations of the problem of suicide ( condition in the Splitz region ) ) .
	manualset3
236950	3	423373	15	NULL	NULL	0	NULL	condition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Epidemiological considerations of the problem of suicide ( condition in the Splitz region ) ) .
	manualset3
236951	4	423373	15	NULL	NULL	0	NULL	Splitz region	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Epidemiological considerations of the problem of suicide ( condition in the Splitz region ) ) .
	manualset3
236952	1	423374	15	NULL	NULL	0	NULL	Analysis of the results	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the results indicates that immunoglobulins detectable on the surface of the blast cells in the cited forms of leukemia are antibodies to the antigens of these cells .
	manualset3
236953	2	423374	15	NULL	NULL	0	NULL	immunoglobulins 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the results indicates that immunoglobulins detectable on the surface of the blast cells in the cited forms of leukemia are antibodies to the antigens of these cells .
	manualset3
236954	3	423374	15	NULL	NULL	0	NULL	blast cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the results indicates that immunoglobulins detectable on the surface of the blast cells in the cited forms of leukemia are antibodies to the antigens of these cells .
	manualset3
236955	4	423374	15	NULL	NULL	0	NULL	leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the results indicates that immunoglobulins detectable on the surface of the blast cells in the cited forms of leukemia are antibodies to the antigens of these cells .
	manualset3
236956	5	423374	15	NULL	NULL	0	NULL	antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the results indicates that immunoglobulins detectable on the surface of the blast cells in the cited forms of leukemia are antibodies to the antigens of these cells .
	manualset3
236957	6	423374	15	NULL	NULL	0	NULL	antigens	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the results indicates that immunoglobulins detectable on the surface of the blast cells in the cited forms of leukemia are antibodies to the antigens of these cells .
	manualset3
236958	7	423374	15	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the results indicates that immunoglobulins detectable on the surface of the blast cells in the cited forms of leukemia are antibodies to the antigens of these cells .
	manualset3
236959	1	423375	15	NULL	NULL	0	NULL	Arterial blood studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterial blood studies revealed that adequate oxygenation is achieved while normal pH and PaCO2 levels are maintained .
	manualset3
236960	2	423375	15	NULL	NULL	0	NULL	oxygenation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterial blood studies revealed that adequate oxygenation is achieved while normal pH and PaCO2 levels are maintained .
	manualset3
236961	3	423375	15	NULL	NULL	0	NULL	pH levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterial blood studies revealed that adequate oxygenation is achieved while normal pH and PaCO2 levels are maintained .
	manualset3
236962	4	423375	15	NULL	NULL	0	NULL	PaCO2 levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterial blood studies revealed that adequate oxygenation is achieved while normal pH and PaCO2 levels are maintained .
	manualset3
236963	1	423376	15	NULL	NULL	0	NULL	historical background	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Against the historical background , the author reviews the current use and future development of arthroscopy .
	manualset3
236964	2	423376	15	NULL	NULL	0	NULL	author	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Against the historical background , the author reviews the current use and future development of arthroscopy .
	manualset3
236965	3	423376	15	NULL	NULL	0	NULL	current use of arthroscopy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Against the historical background , the author reviews the current use and future development of arthroscopy .
	manualset3
236966	4	423376	15	NULL	NULL	0	NULL	future development of arthroscopy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Against the historical background , the author reviews the current use and future development of arthroscopy .
	manualset3
236967	1	423377	15	NULL	NULL	0	NULL	DMXAA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	DMXAA also enhanced the tumor cell killing of cisplatin , but doses ) 15 mg/kg were required .
	manualset3
236968	2	423377	15	NULL	NULL	0	NULL	tumor cell killing 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	DMXAA also enhanced the tumor cell killing of cisplatin , but doses ) 15 mg/kg were required .
	manualset3
236969	3	423377	15	NULL	NULL	0	NULL	cisplatin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	DMXAA also enhanced the tumor cell killing of cisplatin , but doses ) 15 mg/kg were required .
	manualset3
236970	4	423377	15	NULL	NULL	0	NULL	doses 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	DMXAA also enhanced the tumor cell killing of cisplatin , but doses ) 15 mg/kg were required .
	manualset3
236971	5	423377	15	NULL	NULL	0	NULL	15 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	DMXAA also enhanced the tumor cell killing of cisplatin , but doses ) 15 mg/kg were required .
	manualset3
236972	1	423378	15	NULL	NULL	0	NULL	Measurements	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements with extended X-ray adsorption fine structure showed that while the Tc bonding environment in Tris buffer could not be determined , the Tc ( IV ) product in HEPES buffer was very similar to Tc ( IV ) O ( 2 ) nH ( 2 ) O , which was also the product of Tc ( VII ) O ( 4 ) ( - ) reduction by MR-1 cells .
	manualset3
236973	2	423378	15	NULL	NULL	NULL	NULL	X-ray adsorption fine structure	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Measurements with extended X-ray adsorption fine structure showed that while the Tc bonding environment in Tris buffer could not be determined , the Tc ( IV ) product in HEPES buffer was very similar to Tc ( IV ) O ( 2 ) nH ( 2 ) O , which was also the product of Tc ( VII ) O ( 4 ) ( - ) reduction by MR-1 cells .
	manualset3
236974	3	423378	15	NULL	NULL	0	NULL	Tc bonding environment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements with extended X-ray adsorption fine structure showed that while the Tc bonding environment in Tris buffer could not be determined , the Tc ( IV ) product in HEPES buffer was very similar to Tc ( IV ) O ( 2 ) nH ( 2 ) O , which was also the product of Tc ( VII ) O ( 4 ) ( - ) reduction by MR-1 cells .
	manualset3
236975	4	423378	15	NULL	NULL	0	NULL	Tris buffer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements with extended X-ray adsorption fine structure showed that while the Tc bonding environment in Tris buffer could not be determined , the Tc ( IV ) product in HEPES buffer was very similar to Tc ( IV ) O ( 2 ) nH ( 2 ) O , which was also the product of Tc ( VII ) O ( 4 ) ( - ) reduction by MR-1 cells .
	manualset3
237073	5	423378	15	NULL	NULL	0	NULL	Tc ( IV ) product	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements with extended X-ray adsorption fine structure showed that while the Tc bonding environment in Tris buffer could not be determined , the Tc ( IV ) product in HEPES buffer was very similar to Tc ( IV ) O ( 2 ) nH ( 2 ) O , which was also the product of Tc ( VII ) O ( 4 ) ( - ) reduction by MR-1 cells .
	manualset3
237074	6	423378	15	NULL	NULL	0	NULL	HEPES buffer 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements with extended X-ray adsorption fine structure showed that while the Tc bonding environment in Tris buffer could not be determined , the Tc ( IV ) product in HEPES buffer was very similar to Tc ( IV ) O ( 2 ) nH ( 2 ) O , which was also the product of Tc ( VII ) O ( 4 ) ( - ) reduction by MR-1 cells .
	manualset3
237077	7	423378	15	NULL	NULL	0	NULL	Tc ( IV ) O ( 2 ) nH ( 2 ) O	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements with extended X-ray adsorption fine structure showed that while the Tc bonding environment in Tris buffer could not be determined , the Tc ( IV ) product in HEPES buffer was very similar to Tc ( IV ) O ( 2 ) nH ( 2 ) O , which was also the product of Tc ( VII ) O ( 4 ) ( - ) reduction by MR-1 cells .
	manualset3
237081	8	423378	15	NULL	NULL	0	NULL	product	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements with extended X-ray adsorption fine structure showed that while the Tc bonding environment in Tris buffer could not be determined , the Tc ( IV ) product in HEPES buffer was very similar to Tc ( IV ) O ( 2 ) nH ( 2 ) O , which was also the product of Tc ( VII ) O ( 4 ) ( - ) reduction by MR-1 cells .
	manualset3
237084	9	423378	15	NULL	NULL	0	NULL	Tc ( VII ) O ( 4 ) ( - ) reduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements with extended X-ray adsorption fine structure showed that while the Tc bonding environment in Tris buffer could not be determined , the Tc ( IV ) product in HEPES buffer was very similar to Tc ( IV ) O ( 2 ) nH ( 2 ) O , which was also the product of Tc ( VII ) O ( 4 ) ( - ) reduction by MR-1 cells .
	manualset3
237086	10	423378	15	NULL	NULL	0	NULL	MR-1 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Measurements with extended X-ray adsorption fine structure showed that while the Tc bonding environment in Tris buffer could not be determined , the Tc ( IV ) product in HEPES buffer was very similar to Tc ( IV ) O ( 2 ) nH ( 2 ) O , which was also the product of Tc ( VII ) O ( 4 ) ( - ) reduction by MR-1 cells .
	manualset3
237091	1	423379	15	NULL	NULL	0	NULL	Antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies to Tamm-Horsfall protein in patients with acute pyelonephritis .
	manualset3
237093	2	423379	15	NULL	NULL	0	NULL	Tamm-Horsfall protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies to Tamm-Horsfall protein in patients with acute pyelonephritis .
	manualset3
237094	3	423379	15	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies to Tamm-Horsfall protein in patients with acute pyelonephritis .
	manualset3
237101	4	423379	15	NULL	NULL	0	NULL	acute pyelonephritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies to Tamm-Horsfall protein in patients with acute pyelonephritis .
	manualset3
237107	1	423380	15	NULL	NULL	0	NULL	lower concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	At much lower concentrations , the nonapeptide severely inhibited mating .
	manualset3
237109	2	423380	15	NULL	NULL	0	NULL	nonapeptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	At much lower concentrations , the nonapeptide severely inhibited mating .
	manualset3
237113	3	423380	15	NULL	NULL	0	NULL	 mating	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	At much lower concentrations , the nonapeptide severely inhibited mating .
	manualset3
237159	1	423381	15	NULL	NULL	0	NULL	equation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	An equation was derived of the form : T - Au1k1u2 -- k2 where u1 end u2 are the aerobic and anaerobic fractions respectively which has been found to yield highly significant correlation coefficient between log-estimated and log-observed endurance time ( 0.9996 for Astrand and Rodahl 's data on a single subject and 0.9640 for the present data on 13 subjects ) .
	manualset3
237181	2	423381	15	NULL	NULL	0	NULL	form : T - Au1k1u2 -- k2	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	An equation was derived of the form : T - Au1k1u2 -- k2 where u1 end u2 are the aerobic and anaerobic fractions respectively which has been found to yield highly significant correlation coefficient between log-estimated and log-observed endurance time ( 0.9996 for Astrand and Rodahl 's data on a single subject and 0.9640 for the present data on 13 subjects ) .
	manualset3
237184	3	423381	15	NULL	NULL	0	NULL	u1 end u2 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	An equation was derived of the form : T - Au1k1u2 -- k2 where u1 end u2 are the aerobic and anaerobic fractions respectively which has been found to yield highly significant correlation coefficient between log-estimated and log-observed endurance time ( 0.9996 for Astrand and Rodahl 's data on a single subject and 0.9640 for the present data on 13 subjects ) .
	manualset3
237185	4	423381	15	NULL	NULL	0	NULL	aerobic fractions	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	An equation was derived of the form : T - Au1k1u2 -- k2 where u1 end u2 are the aerobic and anaerobic fractions respectively which has been found to yield highly significant correlation coefficient between log-estimated and log-observed endurance time ( 0.9996 for Astrand and Rodahl 's data on a single subject and 0.9640 for the present data on 13 subjects ) .
	manualset3
237186	5	423381	15	NULL	NULL	0	NULL	anaerobic fractions	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	An equation was derived of the form : T - Au1k1u2 -- k2 where u1 end u2 are the aerobic and anaerobic fractions respectively which has been found to yield highly significant correlation coefficient between log-estimated and log-observed endurance time ( 0.9996 for Astrand and Rodahl 's data on a single subject and 0.9640 for the present data on 13 subjects ) .
	manualset3
237187	6	423381	15	NULL	NULL	0	NULL	yield	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An equation was derived of the form : T - Au1k1u2 -- k2 where u1 end u2 are the aerobic and anaerobic fractions respectively which has been found to yield highly significant correlation coefficient between log-estimated and log-observed endurance time ( 0.9996 for Astrand and Rodahl 's data on a single subject and 0.9640 for the present data on 13 subjects ) .
	manualset3
237188	7	423381	15	NULL	NULL	0	NULL	correlation coefficient	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	An equation was derived of the form : T - Au1k1u2 -- k2 where u1 end u2 are the aerobic and anaerobic fractions respectively which has been found to yield highly significant correlation coefficient between log-estimated and log-observed endurance time ( 0.9996 for Astrand and Rodahl 's data on a single subject and 0.9640 for the present data on 13 subjects ) .
	manualset3
237189	8	423381	15	NULL	NULL	0	NULL	log-estimated endurance time	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	An equation was derived of the form : T - Au1k1u2 -- k2 where u1 end u2 are the aerobic and anaerobic fractions respectively which has been found to yield highly significant correlation coefficient between log-estimated and log-observed endurance time ( 0.9996 for Astrand and Rodahl 's data on a single subject and 0.9640 for the present data on 13 subjects ) .
	manualset3
237190	9	423381	15	NULL	NULL	0	NULL	log-observed endurance time	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	An equation was derived of the form : T - Au1k1u2 -- k2 where u1 end u2 are the aerobic and anaerobic fractions respectively which has been found to yield highly significant correlation coefficient between log-estimated and log-observed endurance time ( 0.9996 for Astrand and Rodahl 's data on a single subject and 0.9640 for the present data on 13 subjects ) .
	manualset3
237191	10	423381	15	NULL	NULL	0	NULL	0.9996	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An equation was derived of the form : T - Au1k1u2 -- k2 where u1 end u2 are the aerobic and anaerobic fractions respectively which has been found to yield highly significant correlation coefficient between log-estimated and log-observed endurance time ( 0.9996 for Astrand and Rodahl 's data on a single subject and 0.9640 for the present data on 13 subjects ) .
	manualset3
237192	11	423381	15	NULL	NULL	NULL	NULL	Astrand data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An equation was derived of the form : T - Au1k1u2 -- k2 where u1 end u2 are the aerobic and anaerobic fractions respectively which has been found to yield highly significant correlation coefficient between log-estimated and log-observed endurance time ( 0.9996 for Astrand and Rodahl 's data on a single subject and 0.9640 for the present data on 13 subjects ) .
	manualset3
237193	12	423381	15	NULL	NULL	NULL	NULL	Rodahl 's data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An equation was derived of the form : T - Au1k1u2 -- k2 where u1 end u2 are the aerobic and anaerobic fractions respectively which has been found to yield highly significant correlation coefficient between log-estimated and log-observed endurance time ( 0.9996 for Astrand and Rodahl 's data on a single subject and 0.9640 for the present data on 13 subjects ) .
	manualset3
237194	13	423381	15	NULL	NULL	0	NULL	subject	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	An equation was derived of the form : T - Au1k1u2 -- k2 where u1 end u2 are the aerobic and anaerobic fractions respectively which has been found to yield highly significant correlation coefficient between log-estimated and log-observed endurance time ( 0.9996 for Astrand and Rodahl 's data on a single subject and 0.9640 for the present data on 13 subjects ) .
	manualset3
237195	14	423381	15	NULL	NULL	0	NULL	0.9640	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An equation was derived of the form : T - Au1k1u2 -- k2 where u1 end u2 are the aerobic and anaerobic fractions respectively which has been found to yield highly significant correlation coefficient between log-estimated and log-observed endurance time ( 0.9996 for Astrand and Rodahl 's data on a single subject and 0.9640 for the present data on 13 subjects ) .
	manualset3
237196	15	423381	15	NULL	NULL	NULL	NULL	present data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	An equation was derived of the form : T - Au1k1u2 -- k2 where u1 end u2 are the aerobic and anaerobic fractions respectively which has been found to yield highly significant correlation coefficient between log-estimated and log-observed endurance time ( 0.9996 for Astrand and Rodahl 's data on a single subject and 0.9640 for the present data on 13 subjects ) .
	manualset3
237197	16	423381	15	NULL	NULL	0	NULL	13 subjects	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	An equation was derived of the form : T - Au1k1u2 -- k2 where u1 end u2 are the aerobic and anaerobic fractions respectively which has been found to yield highly significant correlation coefficient between log-estimated and log-observed endurance time ( 0.9996 for Astrand and Rodahl 's data on a single subject and 0.9640 for the present data on 13 subjects ) .
	manualset3
237116	1	423382	15	NULL	NULL	0	NULL	protective effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The protective effects of Clostridium sordellii lethal toxin ( LT ) and hemorrhagic toxin ( HT ) toxoids against challenge with spores in guinea pigs were investigated .
	manualset3
237120	2	423382	15	NULL	NULL	0	NULL	Clostridium sordellii lethal toxin ( LT )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The protective effects of Clostridium sordellii lethal toxin ( LT ) and hemorrhagic toxin ( HT ) toxoids against challenge with spores in guinea pigs were investigated .
	manualset3
237126	3	423382	15	NULL	NULL	0	NULL	hemorrhagic toxin ( HT ) toxoids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The protective effects of Clostridium sordellii lethal toxin ( LT ) and hemorrhagic toxin ( HT ) toxoids against challenge with spores in guinea pigs were investigated .
	manualset3
237129	4	423382	15	NULL	NULL	0	NULL	challenge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The protective effects of Clostridium sordellii lethal toxin ( LT ) and hemorrhagic toxin ( HT ) toxoids against challenge with spores in guinea pigs were investigated .
	manualset3
237144	5	423382	15	NULL	NULL	0	NULL	spores 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The protective effects of Clostridium sordellii lethal toxin ( LT ) and hemorrhagic toxin ( HT ) toxoids against challenge with spores in guinea pigs were investigated .
	manualset3
237145	6	423382	15	NULL	NULL	0	NULL	guinea pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The protective effects of Clostridium sordellii lethal toxin ( LT ) and hemorrhagic toxin ( HT ) toxoids against challenge with spores in guinea pigs were investigated .
	manualset3
237146	1	423383	15	NULL	NULL	NULL	NULL	Analysis of the structure 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Analysis of the structure of T4 bacteriophage-modified valyl-tRNA synthetase by limited proteolysis and isoelectric focusing .
	manualset3
237150	2	423383	15	NULL	NULL	0	NULL	T4 bacteriophage-modified valyl-tRNA synthetase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the structure of T4 bacteriophage-modified valyl-tRNA synthetase by limited proteolysis and isoelectric focusing .
	manualset3
237153	3	423383	15	NULL	NULL	NULL	NULL	limited proteolysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Analysis of the structure of T4 bacteriophage-modified valyl-tRNA synthetase by limited proteolysis and isoelectric focusing .
	manualset3
237156	4	423383	15	NULL	NULL	0	NULL	 isoelectric focusing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the structure of T4 bacteriophage-modified valyl-tRNA synthetase by limited proteolysis and isoelectric focusing .
	manualset3
237203	1	423384	15	NULL	NULL	0	NULL	part 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	It takes part in cell autolysis , separation of daughter cells , biofilm formation , fibronectin-binding activity , cell adhesion , and pathogenesis of HA9801 .
	manualset3
237204	2	423384	15	NULL	NULL	0	NULL	cell autolysis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It takes part in cell autolysis , separation of daughter cells , biofilm formation , fibronectin-binding activity , cell adhesion , and pathogenesis of HA9801 .
	manualset3
237205	3	423384	15	NULL	NULL	0	NULL	separation of daughter cells	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It takes part in cell autolysis , separation of daughter cells , biofilm formation , fibronectin-binding activity , cell adhesion , and pathogenesis of HA9801 .
	manualset3
237206	4	423384	15	NULL	NULL	0	NULL	biofilm formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It takes part in cell autolysis , separation of daughter cells , biofilm formation , fibronectin-binding activity , cell adhesion , and pathogenesis of HA9801 .
	manualset3
237207	5	423384	15	NULL	NULL	0	NULL	fibronectin-binding activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It takes part in cell autolysis , separation of daughter cells , biofilm formation , fibronectin-binding activity , cell adhesion , and pathogenesis of HA9801 .
	manualset3
237208	6	423384	15	NULL	NULL	0	NULL	cell adhesion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It takes part in cell autolysis , separation of daughter cells , biofilm formation , fibronectin-binding activity , cell adhesion , and pathogenesis of HA9801 .
	manualset3
237209	7	423384	15	NULL	NULL	0	NULL	pathogenesis of HA9801	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	It takes part in cell autolysis , separation of daughter cells , biofilm formation , fibronectin-binding activity , cell adhesion , and pathogenesis of HA9801 .
	manualset3
237517	1	423385	15	NULL	NULL	0	NULL	region 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	An intrinsically disordered region often folds in different structures allowing an IDP to recognize and bind different partners at various binding interfaces .
	manualset3
237518	2	423385	15	NULL	NULL	0	NULL	structures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	An intrinsically disordered region often folds in different structures allowing an IDP to recognize and bind different partners at various binding interfaces .
	manualset3
237519	3	423385	15	NULL	NULL	0	NULL	IDP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	An intrinsically disordered region often folds in different structures allowing an IDP to recognize and bind different partners at various binding interfaces .
	manualset3
237520	4	423385	15	NULL	NULL	0	NULL	partners	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	An intrinsically disordered region often folds in different structures allowing an IDP to recognize and bind different partners at various binding interfaces .
	manualset3
237521	1	423386	15	NULL	NULL	0	NULL	case	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	We report herein the unusual case of a 19-year-old , otherwise healthy woman with no history of liver disease who presented with upper abdominal pain and hepatomegaly .
	manualset3
237522	2	423386	15	NULL	NULL	0	NULL	19-year-old 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	We report herein the unusual case of a 19-year-old , otherwise healthy woman with no history of liver disease who presented with upper abdominal pain and hepatomegaly .
	manualset3
237523	3	423386	15	NULL	NULL	0	NULL	woman	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	We report herein the unusual case of a 19-year-old , otherwise healthy woman with no history of liver disease who presented with upper abdominal pain and hepatomegaly .
	manualset3
237524	4	423386	15	NULL	NULL	0	NULL	history	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	We report herein the unusual case of a 19-year-old , otherwise healthy woman with no history of liver disease who presented with upper abdominal pain and hepatomegaly .
	manualset3
237525	5	423386	15	NULL	NULL	0	NULL	liver disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	We report herein the unusual case of a 19-year-old , otherwise healthy woman with no history of liver disease who presented with upper abdominal pain and hepatomegaly .
	manualset3
237526	6	423386	15	NULL	NULL	0	NULL	upper abdominal pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We report herein the unusual case of a 19-year-old , otherwise healthy woman with no history of liver disease who presented with upper abdominal pain and hepatomegaly .
	manualset3
237527	7	423386	15	NULL	NULL	0	NULL	hepatomegaly	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	We report herein the unusual case of a 19-year-old , otherwise healthy woman with no history of liver disease who presented with upper abdominal pain and hepatomegaly .
	manualset3
237528	1	423387	15	NULL	NULL	0	NULL	 depolarization	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This depolarization , characterized by potassium ( K + ) efflux and calcium ( Ca + + ) influx , results in membrane destabilization , osmotic imbalance , and a decrease in electrical conduction .
	manualset3
237529	2	423387	15	NULL	NULL	0	NULL	potassium ( K + ) efflux	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This depolarization , characterized by potassium ( K + ) efflux and calcium ( Ca + + ) influx , results in membrane destabilization , osmotic imbalance , and a decrease in electrical conduction .
	manualset3
237530	3	423387	15	NULL	NULL	0	NULL	calcium ( Ca + + ) influx	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This depolarization , characterized by potassium ( K + ) efflux and calcium ( Ca + + ) influx , results in membrane destabilization , osmotic imbalance , and a decrease in electrical conduction .
	manualset3
237531	4	423387	15	NULL	NULL	0	NULL	membrane destabilization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This depolarization , characterized by potassium ( K + ) efflux and calcium ( Ca + + ) influx , results in membrane destabilization , osmotic imbalance , and a decrease in electrical conduction .
	manualset3
237532	5	423387	15	NULL	NULL	0	NULL	osmotic imbalance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This depolarization , characterized by potassium ( K + ) efflux and calcium ( Ca + + ) influx , results in membrane destabilization , osmotic imbalance , and a decrease in electrical conduction .
	manualset3
237533	6	423387	15	NULL	NULL	0	NULL	decrease in electrical conduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	This depolarization , characterized by potassium ( K + ) efflux and calcium ( Ca + + ) influx , results in membrane destabilization , osmotic imbalance , and a decrease in electrical conduction .
	manualset3
237534	1	423388	15	NULL	NULL	NULL	NULL	complement 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As a complement to these analyses , the implementation of a given neuroscientific hypothesis on a real mechanical system could overcome these measurement artifact and provide a tool that is , under full control of the experimenter , able to replicate the relevant functional features of the human arm .
	manualset3
237535	2	423388	15	NULL	NULL	0	NULL	analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	As a complement to these analyses , the implementation of a given neuroscientific hypothesis on a real mechanical system could overcome these measurement artifact and provide a tool that is , under full control of the experimenter , able to replicate the relevant functional features of the human arm .
	manualset3
237536	3	423388	15	NULL	NULL	0	NULL	implementation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As a complement to these analyses , the implementation of a given neuroscientific hypothesis on a real mechanical system could overcome these measurement artifact and provide a tool that is , under full control of the experimenter , able to replicate the relevant functional features of the human arm .
	manualset3
237537	4	423388	15	NULL	NULL	0	NULL	neuroscientific hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	As a complement to these analyses , the implementation of a given neuroscientific hypothesis on a real mechanical system could overcome these measurement artifact and provide a tool that is , under full control of the experimenter , able to replicate the relevant functional features of the human arm .
	manualset3
237538	5	423388	15	NULL	NULL	0	NULL	mechanical system	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As a complement to these analyses , the implementation of a given neuroscientific hypothesis on a real mechanical system could overcome these measurement artifact and provide a tool that is , under full control of the experimenter , able to replicate the relevant functional features of the human arm .
	manualset3
237539	6	423388	15	NULL	NULL	NULL	NULL	measurement artifact	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As a complement to these analyses , the implementation of a given neuroscientific hypothesis on a real mechanical system could overcome these measurement artifact and provide a tool that is , under full control of the experimenter , able to replicate the relevant functional features of the human arm .
	manualset3
237540	7	423388	15	NULL	NULL	0	NULL	tool 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	As a complement to these analyses , the implementation of a given neuroscientific hypothesis on a real mechanical system could overcome these measurement artifact and provide a tool that is , under full control of the experimenter , able to replicate the relevant functional features of the human arm .
	manualset3
237541	8	423388	15	NULL	NULL	0	NULL	full control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As a complement to these analyses , the implementation of a given neuroscientific hypothesis on a real mechanical system could overcome these measurement artifact and provide a tool that is , under full control of the experimenter , able to replicate the relevant functional features of the human arm .
	manualset3
237542	9	423388	15	NULL	NULL	0	NULL	experimenter	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	As a complement to these analyses , the implementation of a given neuroscientific hypothesis on a real mechanical system could overcome these measurement artifact and provide a tool that is , under full control of the experimenter , able to replicate the relevant functional features of the human arm .
	manualset3
237543	10	423388	15	NULL	NULL	NULL	NULL	functional features	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As a complement to these analyses , the implementation of a given neuroscientific hypothesis on a real mechanical system could overcome these measurement artifact and provide a tool that is , under full control of the experimenter , able to replicate the relevant functional features of the human arm .
	manualset3
237544	11	423388	15	NULL	NULL	0	NULL	human arm	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	As a complement to these analyses , the implementation of a given neuroscientific hypothesis on a real mechanical system could overcome these measurement artifact and provide a tool that is , under full control of the experimenter , able to replicate the relevant functional features of the human arm .
	manualset3
237545	1	423389	15	NULL	NULL	0	NULL	Analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the temporal pattern of haemagglutinin clade data shows a progression from clade 0 ( the ` dominant ' clade between 1996 and 2002 ) to clade 1 ( 2003-2005 ) and then to clade 2.3.4 ( 2005 onwards ) .
	manualset3
237546	2	423389	15	NULL	NULL	NULL	NULL	temporal pattern of haemagglutinin clade data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Analysis of the temporal pattern of haemagglutinin clade data shows a progression from clade 0 ( the ` dominant ' clade between 1996 and 2002 ) to clade 1 ( 2003-2005 ) and then to clade 2.3.4 ( 2005 onwards ) .
	manualset3
237547	3	423389	15	NULL	NULL	0	NULL	progression 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the temporal pattern of haemagglutinin clade data shows a progression from clade 0 ( the ` dominant ' clade between 1996 and 2002 ) to clade 1 ( 2003-2005 ) and then to clade 2.3.4 ( 2005 onwards ) .
	manualset3
237548	4	423389	15	NULL	NULL	NULL	NULL	clade 0	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Analysis of the temporal pattern of haemagglutinin clade data shows a progression from clade 0 ( the ` dominant ' clade between 1996 and 2002 ) to clade 1 ( 2003-2005 ) and then to clade 2.3.4 ( 2005 onwards ) .
	manualset3
237549	5	423389	15	NULL	NULL	0	NULL	clade	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the temporal pattern of haemagglutinin clade data shows a progression from clade 0 ( the ` dominant ' clade between 1996 and 2002 ) to clade 1 ( 2003-2005 ) and then to clade 2.3.4 ( 2005 onwards ) .
	manualset3
237550	6	423389	15	NULL	NULL	0	NULL	1996 and 2002	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the temporal pattern of haemagglutinin clade data shows a progression from clade 0 ( the ` dominant ' clade between 1996 and 2002 ) to clade 1 ( 2003-2005 ) and then to clade 2.3.4 ( 2005 onwards ) .
	manualset3
237551	7	423389	15	NULL	NULL	0	NULL	clade 1	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the temporal pattern of haemagglutinin clade data shows a progression from clade 0 ( the ` dominant ' clade between 1996 and 2002 ) to clade 1 ( 2003-2005 ) and then to clade 2.3.4 ( 2005 onwards ) .
	manualset3
237552	8	423389	15	NULL	NULL	0	NULL	2003-2005	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the temporal pattern of haemagglutinin clade data shows a progression from clade 0 ( the ` dominant ' clade between 1996 and 2002 ) to clade 1 ( 2003-2005 ) and then to clade 2.3.4 ( 2005 onwards ) .
	manualset3
237553	9	423389	15	NULL	NULL	0	NULL	clade 2.3.4	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the temporal pattern of haemagglutinin clade data shows a progression from clade 0 ( the ` dominant ' clade between 1996 and 2002 ) to clade 1 ( 2003-2005 ) and then to clade 2.3.4 ( 2005 onwards ) .
	manualset3
237554	10	423389	15	NULL	NULL	0	NULL	2005 onwards	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of the temporal pattern of haemagglutinin clade data shows a progression from clade 0 ( the ` dominant ' clade between 1996 and 2002 ) to clade 1 ( 2003-2005 ) and then to clade 2.3.4 ( 2005 onwards ) .
	manualset3
237555	1	423390	15	NULL	NULL	0	NULL	Gel filtration analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Gel filtration analysis revealed that PolyP supported the formation of homodimers of PPGK and that PPGK was active as a homodimer .
	manualset3
237556	2	423390	15	NULL	NULL	0	NULL	PolyP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Gel filtration analysis revealed that PolyP supported the formation of homodimers of PPGK and that PPGK was active as a homodimer .
	manualset3
237557	3	423390	15	NULL	NULL	0	NULL	formation of homodimers of PPGK	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Gel filtration analysis revealed that PolyP supported the formation of homodimers of PPGK and that PPGK was active as a homodimer .
	manualset3
237558	4	423390	15	NULL	NULL	0	NULL	PPGK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Gel filtration analysis revealed that PolyP supported the formation of homodimers of PPGK and that PPGK was active as a homodimer .
	manualset3
237559	5	423390	15	NULL	NULL	NULL	NULL	homodimer 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Gel filtration analysis revealed that PolyP supported the formation of homodimers of PPGK and that PPGK was active as a homodimer .
	manualset3
237560	1	423391	15	NULL	NULL	0	NULL	Taurine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Taurine as well as uric acid partially prevented the activity loss from ozone exposure .
	manualset3
237561	2	423391	15	NULL	NULL	0	NULL	uric acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Taurine as well as uric acid partially prevented the activity loss from ozone exposure .
	manualset3
237562	3	423391	15	NULL	NULL	0	NULL	activity loss	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Taurine as well as uric acid partially prevented the activity loss from ozone exposure .
	manualset3
237563	4	423391	15	NULL	NULL	0	NULL	ozone exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Taurine as well as uric acid partially prevented the activity loss from ozone exposure .
	manualset3
237564	1	423392	15	NULL	NULL	0	NULL	analytically relevant units	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	All analytically relevant units are integrated on a microchip ( microreactor , control electrode , glucose oxidase based sensor electrode , reference electrode , counter electrode ) .
	manualset3
237565	2	423392	15	NULL	NULL	0	NULL	microchip	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	All analytically relevant units are integrated on a microchip ( microreactor , control electrode , glucose oxidase based sensor electrode , reference electrode , counter electrode ) .
	manualset3
237566	3	423392	15	NULL	NULL	NULL	NULL	microreactor	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	All analytically relevant units are integrated on a microchip ( microreactor , control electrode , glucose oxidase based sensor electrode , reference electrode , counter electrode ) .
	manualset3
237567	4	423392	15	NULL	NULL	NULL	NULL	control electrode	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	All analytically relevant units are integrated on a microchip ( microreactor , control electrode , glucose oxidase based sensor electrode , reference electrode , counter electrode ) .
	manualset3
237568	5	423392	15	NULL	NULL	NULL	NULL	glucose oxidase based sensor electrode	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	All analytically relevant units are integrated on a microchip ( microreactor , control electrode , glucose oxidase based sensor electrode , reference electrode , counter electrode ) .
	manualset3
237569	6	423392	15	NULL	NULL	0	NULL	reference electrode	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	All analytically relevant units are integrated on a microchip ( microreactor , control electrode , glucose oxidase based sensor electrode , reference electrode , counter electrode ) .
	manualset3
237570	7	423392	15	NULL	NULL	0	NULL	counter electrode	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	All analytically relevant units are integrated on a microchip ( microreactor , control electrode , glucose oxidase based sensor electrode , reference electrode , counter electrode ) .
	manualset3
237571	1	423393	15	NULL	NULL	0	NULL	Nogo-B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nogo-B is phosphorylated at Ser107 in vitro by MAPKAP-K2 ( MAPK ( mitogen-activated protein kinase ) - activated protein kinase-2 ) or MAPKAP-K3 , but not by other protein kinases that are known to be activated by SAPK2a/p38a .
	manualset3
237572	2	423393	15	NULL	NULL	0	NULL	Ser107	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Nogo-B is phosphorylated at Ser107 in vitro by MAPKAP-K2 ( MAPK ( mitogen-activated protein kinase ) - activated protein kinase-2 ) or MAPKAP-K3 , but not by other protein kinases that are known to be activated by SAPK2a/p38a .
	manualset3
237573	3	423393	15	NULL	NULL	NULL	NULL	MAPKAP-K2 ( MAPK ( mitogen-activated protein kinase ) - activated protein kinase-2 )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Nogo-B is phosphorylated at Ser107 in vitro by MAPKAP-K2 ( MAPK ( mitogen-activated protein kinase ) - activated protein kinase-2 ) or MAPKAP-K3 , but not by other protein kinases that are known to be activated by SAPK2a/p38a .
	manualset3
237574	4	423393	15	NULL	NULL	0	NULL	MAPKAP-K3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nogo-B is phosphorylated at Ser107 in vitro by MAPKAP-K2 ( MAPK ( mitogen-activated protein kinase ) - activated protein kinase-2 ) or MAPKAP-K3 , but not by other protein kinases that are known to be activated by SAPK2a/p38a .
	manualset3
237575	5	423393	15	NULL	NULL	0	NULL	protein kinases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Nogo-B is phosphorylated at Ser107 in vitro by MAPKAP-K2 ( MAPK ( mitogen-activated protein kinase ) - activated protein kinase-2 ) or MAPKAP-K3 , but not by other protein kinases that are known to be activated by SAPK2a/p38a .
	manualset3
237576	6	423393	15	NULL	NULL	0	NULL	SAPK2a/p38a	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Nogo-B is phosphorylated at Ser107 in vitro by MAPKAP-K2 ( MAPK ( mitogen-activated protein kinase ) - activated protein kinase-2 ) or MAPKAP-K3 , but not by other protein kinases that are known to be activated by SAPK2a/p38a .
	manualset3
237601	1	423394	15	NULL	NULL	0	NULL	 fumagillin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Although fumagillin and thiabendazole significantly reduced spore counts , in no individual was the pathogen totally eliminated .
	manualset3
237603	2	423394	15	NULL	NULL	0	NULL	thiabendazole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Although fumagillin and thiabendazole significantly reduced spore counts , in no individual was the pathogen totally eliminated .
	manualset3
237604	3	423394	15	NULL	NULL	0	NULL	spore counts	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Although fumagillin and thiabendazole significantly reduced spore counts , in no individual was the pathogen totally eliminated .
	manualset3
237605	4	423394	15	NULL	NULL	0	NULL	pathogen	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Although fumagillin and thiabendazole significantly reduced spore counts , in no individual was the pathogen totally eliminated .
	manualset3
237611	1	423395	15	NULL	NULL	0	NULL	right ventricular papillary muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	In right ventricular papillary muscles , 30 microM MTO increased isometric force of contraction as well as action potential duration ( APD ) in a time-dependent manner .
	manualset3
237621	2	423395	15	NULL	NULL	0	NULL	30 microM MTO	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	In right ventricular papillary muscles , 30 microM MTO increased isometric force of contraction as well as action potential duration ( APD ) in a time-dependent manner .
	manualset3
237623	3	423395	15	NULL	NULL	NULL	NULL	isometric force of contraction	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In right ventricular papillary muscles , 30 microM MTO increased isometric force of contraction as well as action potential duration ( APD ) in a time-dependent manner .
	manualset3
237632	4	423395	15	NULL	NULL	0	NULL	action potential duration ( APD )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	In right ventricular papillary muscles , 30 microM MTO increased isometric force of contraction as well as action potential duration ( APD ) in a time-dependent manner .
	manualset3
237633	5	423395	15	NULL	NULL	NULL	NULL	time-dependent manner	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	In right ventricular papillary muscles , 30 microM MTO increased isometric force of contraction as well as action potential duration ( APD ) in a time-dependent manner .
	manualset3
237644	1	423396	15	NULL	NULL	0	NULL	Neuroendocrine ( Merkel cell ) tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroendocrine ( Merkel cell ) tumor of the skin : fine-needle aspiration cytology , histology , electron microscopy and immunohistochemistry of 12 cases .
	manualset3
237645	2	423396	15	NULL	NULL	0	NULL	skin	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroendocrine ( Merkel cell ) tumor of the skin : fine-needle aspiration cytology , histology , electron microscopy and immunohistochemistry of 12 cases .
	manualset3
237646	3	423396	15	NULL	NULL	0	NULL	fine-needle aspiration cytology	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroendocrine ( Merkel cell ) tumor of the skin : fine-needle aspiration cytology , histology , electron microscopy and immunohistochemistry of 12 cases .
	manualset3
237647	4	423396	15	NULL	NULL	0	NULL	histology 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroendocrine ( Merkel cell ) tumor of the skin : fine-needle aspiration cytology , histology , electron microscopy and immunohistochemistry of 12 cases .
	manualset3
237648	5	423396	15	NULL	NULL	0	NULL	electron microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroendocrine ( Merkel cell ) tumor of the skin : fine-needle aspiration cytology , histology , electron microscopy and immunohistochemistry of 12 cases .
	manualset3
237649	6	423396	15	NULL	NULL	0	NULL	 immunohistochemistry 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroendocrine ( Merkel cell ) tumor of the skin : fine-needle aspiration cytology , histology , electron microscopy and immunohistochemistry of 12 cases .
	manualset3
237652	7	423396	15	NULL	NULL	0	NULL	12 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Neuroendocrine ( Merkel cell ) tumor of the skin : fine-needle aspiration cytology , histology , electron microscopy and immunohistochemistry of 12 cases .
	manualset3
237658	1	423397	15	NULL	NULL	0	NULL	oscillations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The oscillations occurred at a rate of 0.9 / min , gradually decreasing in amplitude within 15 min of secretagogue administration .
	manualset3
237659	2	423397	15	NULL	NULL	NULL	NULL	rate of 0.9 / min	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The oscillations occurred at a rate of 0.9 / min , gradually decreasing in amplitude within 15 min of secretagogue administration .
	manualset3
237662	3	423397	15	NULL	NULL	0	NULL	amplitude 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The oscillations occurred at a rate of 0.9 / min , gradually decreasing in amplitude within 15 min of secretagogue administration .
	manualset3
237664	4	423397	15	NULL	NULL	0	NULL	15 min 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The oscillations occurred at a rate of 0.9 / min , gradually decreasing in amplitude within 15 min of secretagogue administration .
	manualset3
237686	5	423397	15	NULL	NULL	0	NULL	secretagogue administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The oscillations occurred at a rate of 0.9 / min , gradually decreasing in amplitude within 15 min of secretagogue administration .
	manualset3
237691	1	423398	15	NULL	NULL	0	NULL	Analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of these one-hour interactions revealed no significant difference between the two groups on measures of comprehension skills .
	manualset3
237694	2	423398	15	NULL	NULL	0	NULL	one-hour interactions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of these one-hour interactions revealed no significant difference between the two groups on measures of comprehension skills .
	manualset3
237707	3	423398	15	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of these one-hour interactions revealed no significant difference between the two groups on measures of comprehension skills .
	manualset3
237709	4	423398	15	NULL	NULL	0	NULL	two groups	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of these one-hour interactions revealed no significant difference between the two groups on measures of comprehension skills .
	manualset3
237710	5	423398	15	NULL	NULL	0	NULL	measures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of these one-hour interactions revealed no significant difference between the two groups on measures of comprehension skills .
	manualset3
237718	6	423398	15	NULL	NULL	0	NULL	comprehension skills	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of these one-hour interactions revealed no significant difference between the two groups on measures of comprehension skills .
	manualset3
237720	1	423399	15	NULL	NULL	0	NULL	TNF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	TNF - and TNF - Gene Polymorphism in Saudi Rheumatoid Arthritis Patients .
	manualset3
237721	2	423399	15	NULL	NULL	0	NULL	TNF - Gene Polymorphism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	TNF - and TNF - Gene Polymorphism in Saudi Rheumatoid Arthritis Patients .
	manualset3
237722	3	423399	15	NULL	NULL	0	NULL	Saudi Rheumatoid Arthritis Patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	TNF - and TNF - Gene Polymorphism in Saudi Rheumatoid Arthritis Patients .
	manualset3
237724	1	423400	15	NULL	NULL	0	NULL	Deletion of type I IFN genes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Deletion of type I IFN genes and resistance to apoptosis induced by type I IFNs are common in glioblastoma .
	manualset3
237726	2	423400	15	NULL	NULL	0	NULL	resistance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Deletion of type I IFN genes and resistance to apoptosis induced by type I IFNs are common in glioblastoma .
	manualset3
237729	3	423400	15	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Deletion of type I IFN genes and resistance to apoptosis induced by type I IFNs are common in glioblastoma .
	manualset3
237730	4	423400	15	NULL	NULL	0	NULL	type I IFNs	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Deletion of type I IFN genes and resistance to apoptosis induced by type I IFNs are common in glioblastoma .
	manualset3
237731	5	423400	15	NULL	NULL	0	NULL	glioblastoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Deletion of type I IFN genes and resistance to apoptosis induced by type I IFNs are common in glioblastoma .
	manualset3
237735	1	423401	15	NULL	NULL	0	NULL	SEP	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	SEP as a major chicken kidney metabolite .
	manualset3
237736	2	423401	15	NULL	NULL	0	NULL	chicken kidney metabolite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	SEP as a major chicken kidney metabolite .
	manualset3
237737	1	423402	15	NULL	NULL	0	NULL	side effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The major side effects were development of cataract and gonadal insufficiency .
	manualset3
237738	2	423402	15	NULL	NULL	0	NULL	development of cataract	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The major side effects were development of cataract and gonadal insufficiency .
	manualset3
237739	3	423402	15	NULL	NULL	0	NULL	development of gonadal insufficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The major side effects were development of cataract and gonadal insufficiency .
	manualset3
237740	1	423403	15	NULL	NULL	0	NULL	case	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( A case of ulcerative colitis causing superior sagittal sinus thrombosis ) .
	manualset3
237741	2	423403	15	NULL	NULL	0	NULL	ulcerative colitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( A case of ulcerative colitis causing superior sagittal sinus thrombosis ) .
	manualset3
237743	3	423403	15	NULL	NULL	0	NULL	superior sagittal sinus thrombosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( A case of ulcerative colitis causing superior sagittal sinus thrombosis ) .
	manualset3
237786	1	423404	15	NULL	NULL	0	NULL	Heterophile type	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Heterophile type-specific substances of bacteria .
	manualset3
237795	2	423404	15	NULL	NULL	0	NULL	substances of bacteria	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Heterophile type-specific substances of bacteria .
	manualset3
237796	1	423405	15	NULL	NULL	0	NULL	Analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of these papers shows that these data are controversial and strongly depend on methodology .
	manualset3
237797	2	423405	15	NULL	NULL	0	NULL	papers	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of these papers shows that these data are controversial and strongly depend on methodology .
	manualset3
237798	3	423405	15	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of these papers shows that these data are controversial and strongly depend on methodology .
	manualset3
237803	4	423405	15	NULL	NULL	0	NULL	methodology 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of these papers shows that these data are controversial and strongly depend on methodology .
	manualset3
237809	1	423406	15	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were followed for an average of 22.5 months , permitting an assessment of prognosis .
	manualset3
237811	2	423406	15	NULL	NULL	0	NULL	22.5 months	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were followed for an average of 22.5 months , permitting an assessment of prognosis .
	manualset3
237815	3	423406	15	NULL	NULL	0	NULL	assessment of prognosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The patients were followed for an average of 22.5 months , permitting an assessment of prognosis .
	manualset3
237816	1	423407	15	NULL	NULL	0	NULL	factors	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important factors influencing the occurrence of this type of injury among this group of lambs were the size and age of the lambs , the positioning of the lambs during bolus administration , the relative size of the dosing gun and bolus , and the large number of animals in the group .
	manualset3
237817	2	423407	15	NULL	NULL	0	NULL	occurrence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important factors influencing the occurrence of this type of injury among this group of lambs were the size and age of the lambs , the positioning of the lambs during bolus administration , the relative size of the dosing gun and bolus , and the large number of animals in the group .
	manualset3
237818	3	423407	15	NULL	NULL	0	NULL	type of injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important factors influencing the occurrence of this type of injury among this group of lambs were the size and age of the lambs , the positioning of the lambs during bolus administration , the relative size of the dosing gun and bolus , and the large number of animals in the group .
	manualset3
237821	4	423407	15	NULL	NULL	0	NULL	group of lambs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important factors influencing the occurrence of this type of injury among this group of lambs were the size and age of the lambs , the positioning of the lambs during bolus administration , the relative size of the dosing gun and bolus , and the large number of animals in the group .
	manualset3
237823	5	423407	15	NULL	NULL	0	NULL	size of the lambs	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important factors influencing the occurrence of this type of injury among this group of lambs were the size and age of the lambs , the positioning of the lambs during bolus administration , the relative size of the dosing gun and bolus , and the large number of animals in the group .
	manualset3
237825	6	423407	15	NULL	NULL	0	NULL	age of the lambs	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important factors influencing the occurrence of this type of injury among this group of lambs were the size and age of the lambs , the positioning of the lambs during bolus administration , the relative size of the dosing gun and bolus , and the large number of animals in the group .
	manualset3
237827	7	423407	15	NULL	NULL	0	NULL	positioning of the lambs	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important factors influencing the occurrence of this type of injury among this group of lambs were the size and age of the lambs , the positioning of the lambs during bolus administration , the relative size of the dosing gun and bolus , and the large number of animals in the group .
	manualset3
237828	8	423407	15	NULL	NULL	0	NULL	bolus administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important factors influencing the occurrence of this type of injury among this group of lambs were the size and age of the lambs , the positioning of the lambs during bolus administration , the relative size of the dosing gun and bolus , and the large number of animals in the group .
	manualset3
237829	9	423407	15	NULL	NULL	0	NULL	relative size	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important factors influencing the occurrence of this type of injury among this group of lambs were the size and age of the lambs , the positioning of the lambs during bolus administration , the relative size of the dosing gun and bolus , and the large number of animals in the group .
	manualset3
237831	10	423407	15	NULL	NULL	0	NULL	dosing gun	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important factors influencing the occurrence of this type of injury among this group of lambs were the size and age of the lambs , the positioning of the lambs during bolus administration , the relative size of the dosing gun and bolus , and the large number of animals in the group .
	manualset3
237832	11	423407	15	NULL	NULL	0	NULL	bolus	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important factors influencing the occurrence of this type of injury among this group of lambs were the size and age of the lambs , the positioning of the lambs during bolus administration , the relative size of the dosing gun and bolus , and the large number of animals in the group .
	manualset3
237837	12	423407	15	NULL	NULL	0	NULL	large number of animals	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important factors influencing the occurrence of this type of injury among this group of lambs were the size and age of the lambs , the positioning of the lambs during bolus administration , the relative size of the dosing gun and bolus , and the large number of animals in the group .
	manualset3
237838	13	423407	15	NULL	NULL	0	NULL	 group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The most important factors influencing the occurrence of this type of injury among this group of lambs were the size and age of the lambs , the positioning of the lambs during bolus administration , the relative size of the dosing gun and bolus , and the large number of animals in the group .
	manualset3
237852	1	423408	15	NULL	NULL	0	NULL	Bleeding	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Bleeding from the incised artery of the single vessel ulcer does not decrease over a 10-min interval .
	manualset3
237853	2	423408	15	NULL	NULL	0	NULL	artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Bleeding from the incised artery of the single vessel ulcer does not decrease over a 10-min interval .
	manualset3
237854	3	423408	15	NULL	NULL	0	NULL	single vessel ulcer	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Bleeding from the incised artery of the single vessel ulcer does not decrease over a 10-min interval .
	manualset3
237855	4	423408	15	NULL	NULL	0	NULL	10-min interval	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Bleeding from the incised artery of the single vessel ulcer does not decrease over a 10-min interval .
	manualset3
237857	1	423409	15	NULL	NULL	0	NULL	mapping	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We show schematically how the mapping can be used for Monte Carlo calculations and argue that it should be free from the sign problem .
	manualset3
237860	2	423409	15	NULL	NULL	0	NULL	Monte Carlo calculations	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	We show schematically how the mapping can be used for Monte Carlo calculations and argue that it should be free from the sign problem .
	manualset3
237863	3	423409	15	NULL	NULL	0	NULL	sign problem	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	We show schematically how the mapping can be used for Monte Carlo calculations and argue that it should be free from the sign problem .
	manualset3
237867	1	423410	15	NULL	NULL	0	NULL	instances	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no instances of hemorrhage , fever , or infection which occur as complications of hypertonic saline abortion .
	manualset3
237870	2	423410	15	NULL	NULL	0	NULL	hemorrhage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no instances of hemorrhage , fever , or infection which occur as complications of hypertonic saline abortion .
	manualset3
237873	3	423410	15	NULL	NULL	0	NULL	fever 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no instances of hemorrhage , fever , or infection which occur as complications of hypertonic saline abortion .
	manualset3
237874	4	423410	15	NULL	NULL	0	NULL	infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no instances of hemorrhage , fever , or infection which occur as complications of hypertonic saline abortion .
	manualset3
237875	5	423410	15	NULL	NULL	0	NULL	complications of hypertonic saline abortion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	There were no instances of hemorrhage , fever , or infection which occur as complications of hypertonic saline abortion .
	manualset3
237876	1	423411	15	NULL	NULL	0	NULL	Analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of this subject 's exome readily identified two rare non-synonymous mutations in PKLR gene as the most likely cause of the IHA , although these two mutations had not been documented before in a single individual .
	manualset3
237880	2	423411	15	NULL	NULL	NULL	NULL	subject 's exome	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Analysis of this subject 's exome readily identified two rare non-synonymous mutations in PKLR gene as the most likely cause of the IHA , although these two mutations had not been documented before in a single individual .
	manualset3
237881	3	423411	15	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of this subject 's exome readily identified two rare non-synonymous mutations in PKLR gene as the most likely cause of the IHA , although these two mutations had not been documented before in a single individual .
	manualset3
237882	4	423411	15	NULL	NULL	0	NULL	rare non-synonymous mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of this subject 's exome readily identified two rare non-synonymous mutations in PKLR gene as the most likely cause of the IHA , although these two mutations had not been documented before in a single individual .
	manualset3
237883	5	423411	15	NULL	NULL	0	NULL	PKLR gene 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of this subject 's exome readily identified two rare non-synonymous mutations in PKLR gene as the most likely cause of the IHA , although these two mutations had not been documented before in a single individual .
	manualset3
237884	6	423411	15	NULL	NULL	0	NULL	cause of the IHA	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of this subject 's exome readily identified two rare non-synonymous mutations in PKLR gene as the most likely cause of the IHA , although these two mutations had not been documented before in a single individual .
	manualset3
237885	7	423411	15	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of this subject 's exome readily identified two rare non-synonymous mutations in PKLR gene as the most likely cause of the IHA , although these two mutations had not been documented before in a single individual .
	manualset3
237886	8	423411	15	NULL	NULL	0	NULL	mutations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of this subject 's exome readily identified two rare non-synonymous mutations in PKLR gene as the most likely cause of the IHA , although these two mutations had not been documented before in a single individual .
	manualset3
237887	9	423411	15	NULL	NULL	0	NULL	single individual 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of this subject 's exome readily identified two rare non-synonymous mutations in PKLR gene as the most likely cause of the IHA , although these two mutations had not been documented before in a single individual .
	manualset3
238083	1	423412	15	NULL	NULL	0	NULL	Pharmacokinetic studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetic studies in rats demonstrated that oral absorption of FB642 was variable and may be saturated at the 2000 mg/kg dose level since higher doses failed to produce a further increase in the area under the time concentration curve .
	manualset3
238085	2	423412	15	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetic studies in rats demonstrated that oral absorption of FB642 was variable and may be saturated at the 2000 mg/kg dose level since higher doses failed to produce a further increase in the area under the time concentration curve .
	manualset3
238086	3	423412	15	NULL	NULL	0	NULL	oral absorption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetic studies in rats demonstrated that oral absorption of FB642 was variable and may be saturated at the 2000 mg/kg dose level since higher doses failed to produce a further increase in the area under the time concentration curve .
	manualset3
238090	4	423412	15	NULL	NULL	0	NULL	FB642	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetic studies in rats demonstrated that oral absorption of FB642 was variable and may be saturated at the 2000 mg/kg dose level since higher doses failed to produce a further increase in the area under the time concentration curve .
	manualset3
238094	5	423412	15	NULL	NULL	0	NULL	2000 mg/kg dose level 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetic studies in rats demonstrated that oral absorption of FB642 was variable and may be saturated at the 2000 mg/kg dose level since higher doses failed to produce a further increase in the area under the time concentration curve .
	manualset3
238097	6	423412	15	NULL	NULL	NULL	NULL	doses	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pharmacokinetic studies in rats demonstrated that oral absorption of FB642 was variable and may be saturated at the 2000 mg/kg dose level since higher doses failed to produce a further increase in the area under the time concentration curve .
	manualset3
238103	7	423412	15	NULL	NULL	NULL	NULL	increase	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Pharmacokinetic studies in rats demonstrated that oral absorption of FB642 was variable and may be saturated at the 2000 mg/kg dose level since higher doses failed to produce a further increase in the area under the time concentration curve .
	manualset3
238109	8	423412	15	NULL	NULL	0	NULL	area	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetic studies in rats demonstrated that oral absorption of FB642 was variable and may be saturated at the 2000 mg/kg dose level since higher doses failed to produce a further increase in the area under the time concentration curve .
	manualset3
238110	9	423412	15	NULL	NULL	0	NULL	time concentration curve	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Pharmacokinetic studies in rats demonstrated that oral absorption of FB642 was variable and may be saturated at the 2000 mg/kg dose level since higher doses failed to produce a further increase in the area under the time concentration curve .
	manualset3
238126	1	423413	15	NULL	NULL	0	NULL	periplasmic side	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	On the periplasmic side , we observe the outer periplasmic bottleneck region adopting in all simulations a conformation more open than the TolC wild-type crystal structures until in one run the successive binding of two sodium ions induces the transition to a conformation more closed than any of the available TolC X-ray structures .
	manualset3
238130	2	423413	15	NULL	NULL	0	NULL	outer periplasmic bottleneck region	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	On the periplasmic side , we observe the outer periplasmic bottleneck region adopting in all simulations a conformation more open than the TolC wild-type crystal structures until in one run the successive binding of two sodium ions induces the transition to a conformation more closed than any of the available TolC X-ray structures .
	manualset3
238132	3	423413	15	NULL	NULL	NULL	NULL	simulations	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On the periplasmic side , we observe the outer periplasmic bottleneck region adopting in all simulations a conformation more open than the TolC wild-type crystal structures until in one run the successive binding of two sodium ions induces the transition to a conformation more closed than any of the available TolC X-ray structures .
	manualset3
238133	4	423413	15	NULL	NULL	NULL	NULL	conformation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	On the periplasmic side , we observe the outer periplasmic bottleneck region adopting in all simulations a conformation more open than the TolC wild-type crystal structures until in one run the successive binding of two sodium ions induces the transition to a conformation more closed than any of the available TolC X-ray structures .
	manualset3
238136	5	423413	15	NULL	NULL	0	NULL	TolC wild-type crystal structures	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the periplasmic side , we observe the outer periplasmic bottleneck region adopting in all simulations a conformation more open than the TolC wild-type crystal structures until in one run the successive binding of two sodium ions induces the transition to a conformation more closed than any of the available TolC X-ray structures .
	manualset3
238139	6	423413	15	NULL	NULL	0	NULL	one run	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the periplasmic side , we observe the outer periplasmic bottleneck region adopting in all simulations a conformation more open than the TolC wild-type crystal structures until in one run the successive binding of two sodium ions induces the transition to a conformation more closed than any of the available TolC X-ray structures .
	manualset3
238145	7	423413	15	NULL	NULL	0	NULL	successive binding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the periplasmic side , we observe the outer periplasmic bottleneck region adopting in all simulations a conformation more open than the TolC wild-type crystal structures until in one run the successive binding of two sodium ions induces the transition to a conformation more closed than any of the available TolC X-ray structures .
	manualset3
238147	8	423413	15	NULL	NULL	0	NULL	two sodium ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	On the periplasmic side , we observe the outer periplasmic bottleneck region adopting in all simulations a conformation more open than the TolC wild-type crystal structures until in one run the successive binding of two sodium ions induces the transition to a conformation more closed than any of the available TolC X-ray structures .
	manualset3
238148	9	423413	15	NULL	NULL	0	NULL	transition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	On the periplasmic side , we observe the outer periplasmic bottleneck region adopting in all simulations a conformation more open than the TolC wild-type crystal structures until in one run the successive binding of two sodium ions induces the transition to a conformation more closed than any of the available TolC X-ray structures .
	manualset3
238150	10	423413	15	NULL	NULL	0	NULL	conformation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	On the periplasmic side , we observe the outer periplasmic bottleneck region adopting in all simulations a conformation more open than the TolC wild-type crystal structures until in one run the successive binding of two sodium ions induces the transition to a conformation more closed than any of the available TolC X-ray structures .
	manualset3
238151	11	423413	15	NULL	NULL	0	NULL	TolC X-ray structures	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	On the periplasmic side , we observe the outer periplasmic bottleneck region adopting in all simulations a conformation more open than the TolC wild-type crystal structures until in one run the successive binding of two sodium ions induces the transition to a conformation more closed than any of the available TolC X-ray structures .
	manualset3
238154	1	423414	15	NULL	NULL	0	NULL	Time dependence	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Time dependence of B cell processing and presentation of peptide and native protein antigens .
	manualset3
238155	2	423414	15	NULL	NULL	0	NULL	B cell processing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Time dependence of B cell processing and presentation of peptide and native protein antigens .
	manualset3
238156	3	423414	15	NULL	NULL	0	NULL	presentation of peptide	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Time dependence of B cell processing and presentation of peptide and native protein antigens .
	manualset3
238157	4	423414	15	NULL	NULL	0	NULL	native protein antigens	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Time dependence of B cell processing and presentation of peptide and native protein antigens .
	manualset3
238158	1	423415	15	NULL	NULL	0	NULL	Effect of hypobaric hypoxia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Effect of hypobaric hypoxia on spermatogenesis , Leydig cells and delta 5-3 beta-hydroxysteroid dehydrogenase activity in toad .
	manualset3
238159	2	423415	15	NULL	NULL	0	NULL	spermatogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Effect of hypobaric hypoxia on spermatogenesis , Leydig cells and delta 5-3 beta-hydroxysteroid dehydrogenase activity in toad .
	manualset3
238160	3	423415	15	NULL	NULL	0	NULL	Leydig cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Effect of hypobaric hypoxia on spermatogenesis , Leydig cells and delta 5-3 beta-hydroxysteroid dehydrogenase activity in toad .
	manualset3
238162	4	423415	15	NULL	NULL	0	NULL	delta 5-3 beta-hydroxysteroid dehydrogenase activity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Effect of hypobaric hypoxia on spermatogenesis , Leydig cells and delta 5-3 beta-hydroxysteroid dehydrogenase activity in toad .
	manualset3
238163	5	423415	15	NULL	NULL	0	NULL	toad	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Effect of hypobaric hypoxia on spermatogenesis , Leydig cells and delta 5-3 beta-hydroxysteroid dehydrogenase activity in toad .
	manualset3
238166	1	423416	15	NULL	NULL	0	NULL	program	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This program affords the opportunity to establish whether or not training programs will close the gap between the theory of community participation and actual participation of community members .
	manualset3
238174	2	423416	15	NULL	NULL	0	NULL	opportunity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This program affords the opportunity to establish whether or not training programs will close the gap between the theory of community participation and actual participation of community members .
	manualset3
238178	3	423416	15	NULL	NULL	0	NULL	training programs 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	This program affords the opportunity to establish whether or not training programs will close the gap between the theory of community participation and actual participation of community members .
	manualset3
238184	4	423416	15	NULL	NULL	0	NULL	gap	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	This program affords the opportunity to establish whether or not training programs will close the gap between the theory of community participation and actual participation of community members .
	manualset3
238187	5	423416	15	NULL	NULL	0	NULL	theory of community participation	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This program affords the opportunity to establish whether or not training programs will close the gap between the theory of community participation and actual participation of community members .
	manualset3
238190	6	423416	15	NULL	NULL	0	NULL	theory of actual participation	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	This program affords the opportunity to establish whether or not training programs will close the gap between the theory of community participation and actual participation of community members .
	manualset3
238191	7	423416	15	NULL	NULL	0	NULL	community members	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	This program affords the opportunity to establish whether or not training programs will close the gap between the theory of community participation and actual participation of community members .
	manualset3
238196	1	423417	15	NULL	NULL	0	NULL	cellular proteasome	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The cellular proteasome is an important molecular target in cancer therapy and drug resistance research .
	manualset3
238199	2	423417	15	NULL	NULL	0	NULL	molecular target	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The cellular proteasome is an important molecular target in cancer therapy and drug resistance research .
	manualset3
238200	3	423417	15	NULL	NULL	0	NULL	cancer therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The cellular proteasome is an important molecular target in cancer therapy and drug resistance research .
	manualset3
238201	4	423417	15	NULL	NULL	0	NULL	drug resistance research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The cellular proteasome is an important molecular target in cancer therapy and drug resistance research .
	manualset3
238202	1	423418	15	NULL	NULL	0	NULL	tight junctions 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The tight junctions between the mucosal cells constantly became visible and are considered impermeable ; however , the junctions connecting the mesothelial cells , which face the perilymph , demonstrated high susceptibility against differences in preparation and were structurally different .
	manualset3
238203	2	423418	15	NULL	NULL	0	NULL	mucosal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The tight junctions between the mucosal cells constantly became visible and are considered impermeable ; however , the junctions connecting the mesothelial cells , which face the perilymph , demonstrated high susceptibility against differences in preparation and were structurally different .
	manualset3
238205	3	423418	15	NULL	NULL	0	NULL	junctions	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The tight junctions between the mucosal cells constantly became visible and are considered impermeable ; however , the junctions connecting the mesothelial cells , which face the perilymph , demonstrated high susceptibility against differences in preparation and were structurally different .
	manualset3
238206	4	423418	15	NULL	NULL	0	NULL	mesothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The tight junctions between the mucosal cells constantly became visible and are considered impermeable ; however , the junctions connecting the mesothelial cells , which face the perilymph , demonstrated high susceptibility against differences in preparation and were structurally different .
	manualset3
238207	5	423418	15	NULL	NULL	0	NULL	perilymph	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	The tight junctions between the mucosal cells constantly became visible and are considered impermeable ; however , the junctions connecting the mesothelial cells , which face the perilymph , demonstrated high susceptibility against differences in preparation and were structurally different .
	manualset3
238208	6	423418	15	NULL	NULL	0	NULL	susceptibility 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The tight junctions between the mucosal cells constantly became visible and are considered impermeable ; however , the junctions connecting the mesothelial cells , which face the perilymph , demonstrated high susceptibility against differences in preparation and were structurally different .
	manualset3
238209	7	423418	15	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	The tight junctions between the mucosal cells constantly became visible and are considered impermeable ; however , the junctions connecting the mesothelial cells , which face the perilymph , demonstrated high susceptibility against differences in preparation and were structurally different .
	manualset3
238210	8	423418	15	NULL	NULL	0	NULL	preparation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The tight junctions between the mucosal cells constantly became visible and are considered impermeable ; however , the junctions connecting the mesothelial cells , which face the perilymph , demonstrated high susceptibility against differences in preparation and were structurally different .
	manualset3
238215	1	423419	15	NULL	NULL	0	NULL	Analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of variance performed in 119 neonates of birthweight greater than 2 kg revealed a significant rise with age of both platelet count ( P less than 0.0001 and MPV ( P less than 0.02 ) during the neonatal period .
	manualset3
238219	2	423419	15	NULL	NULL	0	NULL	variance 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of variance performed in 119 neonates of birthweight greater than 2 kg revealed a significant rise with age of both platelet count ( P less than 0.0001 and MPV ( P less than 0.02 ) during the neonatal period .
	manualset3
238221	3	423419	15	NULL	NULL	NULL	NULL	119 neonates	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Analysis of variance performed in 119 neonates of birthweight greater than 2 kg revealed a significant rise with age of both platelet count ( P less than 0.0001 and MPV ( P less than 0.02 ) during the neonatal period .
	manualset3
238224	4	423419	15	NULL	NULL	0	NULL	birthweight	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of variance performed in 119 neonates of birthweight greater than 2 kg revealed a significant rise with age of both platelet count ( P less than 0.0001 and MPV ( P less than 0.02 ) during the neonatal period .
	manualset3
238226	5	423419	15	NULL	NULL	0	NULL	2 kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of variance performed in 119 neonates of birthweight greater than 2 kg revealed a significant rise with age of both platelet count ( P less than 0.0001 and MPV ( P less than 0.02 ) during the neonatal period .
	manualset3
238227	6	423419	15	NULL	NULL	0	NULL	rise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of variance performed in 119 neonates of birthweight greater than 2 kg revealed a significant rise with age of both platelet count ( P less than 0.0001 and MPV ( P less than 0.02 ) during the neonatal period .
	manualset3
238228	7	423419	15	NULL	NULL	0	NULL	age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of variance performed in 119 neonates of birthweight greater than 2 kg revealed a significant rise with age of both platelet count ( P less than 0.0001 and MPV ( P less than 0.02 ) during the neonatal period .
	manualset3
238232	8	423419	15	NULL	NULL	NULL	NULL	platelet count ( P less than 0.0001)	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Analysis of variance performed in 119 neonates of birthweight greater than 2 kg revealed a significant rise with age of both platelet count ( P less than 0.0001 and MPV ( P less than 0.02 ) during the neonatal period .
	manualset3
238233	9	423419	15	NULL	NULL	NULL	NULL	MPV ( P less than 0.02 )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Analysis of variance performed in 119 neonates of birthweight greater than 2 kg revealed a significant rise with age of both platelet count ( P less than 0.0001 and MPV ( P less than 0.02 ) during the neonatal period .
	manualset3
238237	10	423419	15	NULL	NULL	0	NULL	neonatal period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Analysis of variance performed in 119 neonates of birthweight greater than 2 kg revealed a significant rise with age of both platelet count ( P less than 0.0001 and MPV ( P less than 0.02 ) during the neonatal period .
	manualset3
238245	1	423420	15	NULL	NULL	0	NULL	algorithm	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The algorithm achieves high sensitivity and low false positive rates in 10 out of 18 epileptic patients from the Freiburg database .
	manualset3
238246	2	423420	15	NULL	NULL	0	NULL	sensitivity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The algorithm achieves high sensitivity and low false positive rates in 10 out of 18 epileptic patients from the Freiburg database .
	manualset3
238247	3	423420	15	NULL	NULL	0	NULL	false positive rates	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The algorithm achieves high sensitivity and low false positive rates in 10 out of 18 epileptic patients from the Freiburg database .
	manualset3
238248	4	423420	15	NULL	NULL	0	NULL	10 out of 18	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The algorithm achieves high sensitivity and low false positive rates in 10 out of 18 epileptic patients from the Freiburg database .
	manualset3
238249	5	423420	15	NULL	NULL	0	NULL	epileptic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	The algorithm achieves high sensitivity and low false positive rates in 10 out of 18 epileptic patients from the Freiburg database .
	manualset3
238250	6	423420	15	NULL	NULL	0	NULL	Freiburg database	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	The algorithm achieves high sensitivity and low false positive rates in 10 out of 18 epileptic patients from the Freiburg database .
	manualset3
238251	1	423421	15	NULL	NULL	0	NULL	Inactivation of phosphorylase kinase	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of phosphorylase kinase by oATP was sensitive to various effectors of the enzyme such as Ca2 + , Mg2 + , and pH. .
	manualset3
238252	2	423421	15	NULL	NULL	0	NULL	oATP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of phosphorylase kinase by oATP was sensitive to various effectors of the enzyme such as Ca2 + , Mg2 + , and pH. .
	manualset3
238253	3	423421	15	NULL	NULL	0	NULL	effectors of the enzyme	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of phosphorylase kinase by oATP was sensitive to various effectors of the enzyme such as Ca2 + , Mg2 + , and pH. .
	manualset3
238254	4	423421	15	NULL	NULL	0	NULL	Ca2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of phosphorylase kinase by oATP was sensitive to various effectors of the enzyme such as Ca2 + , Mg2 + , and pH. .
	manualset3
238255	5	423421	15	NULL	NULL	0	NULL	Mg2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of phosphorylase kinase by oATP was sensitive to various effectors of the enzyme such as Ca2 + , Mg2 + , and pH. .
	manualset3
238256	6	423421	15	NULL	NULL	0	NULL	pH	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Inactivation of phosphorylase kinase by oATP was sensitive to various effectors of the enzyme such as Ca2 + , Mg2 + , and pH. .
	manualset3
238259	1	423422	15	NULL	NULL	0	NULL	Spreading 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Spreading the word : grass-roots infection education .
	manualset3
238261	2	423422	15	NULL	NULL	0	NULL	word 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Spreading the word : grass-roots infection education .
	manualset3
238262	3	423422	15	NULL	NULL	NULL	NULL	grass-roots infection education	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Spreading the word : grass-roots infection education .
	manualset3
238263	1	423423	15	NULL	NULL	0	NULL	Behavioural observations	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Behavioural observations on the Granville train disaster and the significance of stress for psychiatry .
	manualset3
238264	2	423423	15	NULL	NULL	0	NULL	Granville train disaster	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Behavioural observations on the Granville train disaster and the significance of stress for psychiatry .
	manualset3
238265	3	423423	15	NULL	NULL	0	NULL	significance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Behavioural observations on the Granville train disaster and the significance of stress for psychiatry .
	manualset3
238267	4	423423	15	NULL	NULL	0	NULL	stress 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Behavioural observations on the Granville train disaster and the significance of stress for psychiatry .
	manualset3
238273	5	423423	15	NULL	NULL	0	NULL	psychiatry	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Behavioural observations on the Granville train disaster and the significance of stress for psychiatry .
	manualset3
238279	1	423424	15	NULL	NULL	0	NULL	program	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	The program consisted of an introductory session and three follow-up visits .
	manualset3
238285	2	423424	15	NULL	NULL	0	NULL	session	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The program consisted of an introductory session and three follow-up visits .
	manualset3
238286	3	423424	15	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The program consisted of an introductory session and three follow-up visits .
	manualset3
238289	4	423424	15	NULL	NULL	0	NULL	follow-up visits	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	The program consisted of an introductory session and three follow-up visits .
	manualset3
238294	1	423425	15	NULL	NULL	0	NULL	Biosynthesis of carotenoids	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Biosynthesis and regulation of carotenoids in Dunaliella : progresses and prospects .
	manualset3
238296	2	423425	15	NULL	NULL	0	NULL	regulation of carotenoids	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Biosynthesis and regulation of carotenoids in Dunaliella : progresses and prospects .
	manualset3
238299	3	423425	15	NULL	NULL	0	NULL	Dunaliella	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Biosynthesis and regulation of carotenoids in Dunaliella : progresses and prospects .
	manualset3
238301	4	423425	15	NULL	NULL	0	NULL	 progresses	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Biosynthesis and regulation of carotenoids in Dunaliella : progresses and prospects .
	manualset3
238303	5	423425	15	NULL	NULL	0	NULL	prospects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Biosynthesis and regulation of carotenoids in Dunaliella : progresses and prospects .
	manualset3
238310	1	423426	15	NULL	NULL	0	NULL	beginning of the nineties	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	In the beginning of the nineties an antitoxin had been developed against the so called `` terror of mothers '' .
	manualset3
238311	2	423426	15	NULL	NULL	0	NULL	antitoxin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	In the beginning of the nineties an antitoxin had been developed against the so called `` terror of mothers '' .
	manualset3
238312	3	423426	15	NULL	NULL	0	NULL	terror of mothers	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	In the beginning of the nineties an antitoxin had been developed against the so called `` terror of mothers '' .
	manualset3
238313	1	423427	15	NULL	NULL	0	NULL	percentages of the nodal particles	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentages of the nodal particles that were associated with NMP over the course of the study were inversely proportional to nodal particulate burdens , even though the percentage of cells with engulfed particles increased ; the percentage of NMP asymptotically approached a maximum value over the range of nodal burdens of 6-12 X 10 ( 5 ) particles .
	manualset3
238314	2	423427	15	NULL	NULL	0	NULL	NMP	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentages of the nodal particles that were associated with NMP over the course of the study were inversely proportional to nodal particulate burdens , even though the percentage of cells with engulfed particles increased ; the percentage of NMP asymptotically approached a maximum value over the range of nodal burdens of 6-12 X 10 ( 5 ) particles .
	manualset3
238315	3	423427	15	NULL	NULL	0	NULL	course of the study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The percentages of the nodal particles that were associated with NMP over the course of the study were inversely proportional to nodal particulate burdens , even though the percentage of cells with engulfed particles increased ; the percentage of NMP asymptotically approached a maximum value over the range of nodal burdens of 6-12 X 10 ( 5 ) particles .
	manualset3
238317	4	423427	15	NULL	NULL	NULL	NULL	nodal particulate burdens	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The percentages of the nodal particles that were associated with NMP over the course of the study were inversely proportional to nodal particulate burdens , even though the percentage of cells with engulfed particles increased ; the percentage of NMP asymptotically approached a maximum value over the range of nodal burdens of 6-12 X 10 ( 5 ) particles .
	manualset3
238318	5	423427	15	NULL	NULL	NULL	NULL	percentage of cells	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The percentages of the nodal particles that were associated with NMP over the course of the study were inversely proportional to nodal particulate burdens , even though the percentage of cells with engulfed particles increased ; the percentage of NMP asymptotically approached a maximum value over the range of nodal burdens of 6-12 X 10 ( 5 ) particles .
	manualset3
238319	6	423427	15	NULL	NULL	NULL	NULL	engulfed particles	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The percentages of the nodal particles that were associated with NMP over the course of the study were inversely proportional to nodal particulate burdens , even though the percentage of cells with engulfed particles increased ; the percentage of NMP asymptotically approached a maximum value over the range of nodal burdens of 6-12 X 10 ( 5 ) particles .
	manualset3
238320	7	423427	15	NULL	NULL	NULL	NULL	percentage of NMP	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The percentages of the nodal particles that were associated with NMP over the course of the study were inversely proportional to nodal particulate burdens , even though the percentage of cells with engulfed particles increased ; the percentage of NMP asymptotically approached a maximum value over the range of nodal burdens of 6-12 X 10 ( 5 ) particles .
	manualset3
238321	8	423427	15	NULL	NULL	NULL	NULL	maximum value	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The percentages of the nodal particles that were associated with NMP over the course of the study were inversely proportional to nodal particulate burdens , even though the percentage of cells with engulfed particles increased ; the percentage of NMP asymptotically approached a maximum value over the range of nodal burdens of 6-12 X 10 ( 5 ) particles .
	manualset3
238322	9	423427	15	NULL	NULL	NULL	NULL	range of nodal burdens	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The percentages of the nodal particles that were associated with NMP over the course of the study were inversely proportional to nodal particulate burdens , even though the percentage of cells with engulfed particles increased ; the percentage of NMP asymptotically approached a maximum value over the range of nodal burdens of 6-12 X 10 ( 5 ) particles .
	manualset3
238323	10	423427	15	NULL	NULL	NULL	NULL	6-12 X 10 ( 5 ) particles	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The percentages of the nodal particles that were associated with NMP over the course of the study were inversely proportional to nodal particulate burdens , even though the percentage of cells with engulfed particles increased ; the percentage of NMP asymptotically approached a maximum value over the range of nodal burdens of 6-12 X 10 ( 5 ) particles .
	manualset3
238324	1	423428	15	NULL	NULL	0	NULL	Labor 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Labor complicated by lymphopathia venereum .
	manualset3
238325	2	423428	15	NULL	NULL	0	NULL	lymphopathia venereum	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Labor complicated by lymphopathia venereum .
	manualset3
238326	1	423429	15	NULL	NULL	0	NULL	Severe pulmonary tuberculosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Severe pulmonary tuberculosis after encysted purulent pleurisy ) .
	manualset3
238327	2	423429	15	NULL	NULL	0	NULL	encysted purulent pleurisy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Severe pulmonary tuberculosis after encysted purulent pleurisy ) .
	manualset3
238328	1	423430	15	NULL	NULL	0	NULL	Analytical results	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Analytical and statistical results showed that the concentrations of alkaline earth metals ( except for Mg ) rare earth elements and some heavy metals in D. linearis increased linearly with plant age .
	manualset3
238329	2	423430	15	NULL	NULL	0	NULL	statistical results	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Analytical and statistical results showed that the concentrations of alkaline earth metals ( except for Mg ) rare earth elements and some heavy metals in D. linearis increased linearly with plant age .
	manualset3
238330	3	423430	15	NULL	NULL	0	NULL	concentrations of alkaline earth metals	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Analytical and statistical results showed that the concentrations of alkaline earth metals ( except for Mg ) rare earth elements and some heavy metals in D. linearis increased linearly with plant age .
	manualset3
238331	4	423430	15	NULL	NULL	0	NULL	Mg 	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Analytical and statistical results showed that the concentrations of alkaline earth metals ( except for Mg ) rare earth elements and some heavy metals in D. linearis increased linearly with plant age .
	manualset3
238332	5	423430	15	NULL	NULL	NULL	NULL	rare earth elements	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Analytical and statistical results showed that the concentrations of alkaline earth metals ( except for Mg ) rare earth elements and some heavy metals in D. linearis increased linearly with plant age .
	manualset3
238333	6	423430	15	NULL	NULL	NULL	NULL	heavy metals	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Analytical and statistical results showed that the concentrations of alkaline earth metals ( except for Mg ) rare earth elements and some heavy metals in D. linearis increased linearly with plant age .
	manualset3
238334	7	423430	15	NULL	NULL	0	NULL	D. linearis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Analytical and statistical results showed that the concentrations of alkaline earth metals ( except for Mg ) rare earth elements and some heavy metals in D. linearis increased linearly with plant age .
	manualset3
238335	8	423430	15	NULL	NULL	0	NULL	linearly	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Analytical and statistical results showed that the concentrations of alkaline earth metals ( except for Mg ) rare earth elements and some heavy metals in D. linearis increased linearly with plant age .
	manualset3
238336	9	423430	15	NULL	NULL	0	NULL	plant age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Analytical and statistical results showed that the concentrations of alkaline earth metals ( except for Mg ) rare earth elements and some heavy metals in D. linearis increased linearly with plant age .
	manualset3
238337	2	423431	15	NULL	NULL	NULL	NULL	Mpc-amino acids	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of Mpc-amino acids in solid phase peptide synthesis leads to improved coupling efficiencies .
	manualset3
238338	3	423431	15	NULL	NULL	NULL	NULL	solid phase peptide synthesis	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of Mpc-amino acids in solid phase peptide synthesis leads to improved coupling efficiencies .
	manualset3
238341	4	423431	15	NULL	NULL	NULL	NULL	coupling efficiencies	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of Mpc-amino acids in solid phase peptide synthesis leads to improved coupling efficiencies .
	manualset3
258162	1	423431	15	NULL	NULL	NULL	NULL	Use	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Use of Mpc-amino acids in solid phase peptide synthesis leads to improved coupling efficiencies .
	manualset3
238399	1	423432	15	NULL	NULL	0	NULL	Effect of smoking	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Effect of smoking on benzo ( a ) pyrene metabolism by human placental microsomes .
	manualset3
238400	2	423432	15	NULL	NULL	0	NULL	 benzo ( a ) pyrene metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Effect of smoking on benzo ( a ) pyrene metabolism by human placental microsomes .
	manualset3
238401	3	423432	15	NULL	NULL	0	NULL	human placental microsomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Effect of smoking on benzo ( a ) pyrene metabolism by human placental microsomes .
	manualset3
238402	1	423433	15	NULL	NULL	0	NULL	USQ	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	The USQ correlates positively with physical symptoms and negatively with mood .
	manualset3
238403	2	423433	15	NULL	NULL	0	NULL	physical symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The USQ correlates positively with physical symptoms and negatively with mood .
	manualset3
238404	3	423433	15	NULL	NULL	0	NULL	mood	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The USQ correlates positively with physical symptoms and negatively with mood .
	manualset3
238405	1	423434	15	NULL	NULL	0	NULL	Long-term memory KJ1 .26 ( + ) CD4 ( + ) T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term memory KJ1 .26 ( + ) CD4 ( + ) T cells from wild-type mice were detected in the spleen , lungs and liver during 10 weeks after immunization ; however , Bcl6-deficient KJ1 .26 ( + ) CD4 ( + ) T cells were vanished completely in those organs 4 weeks after immunization .
	manualset3
238406	2	423434	15	NULL	NULL	0	NULL	wild-type mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term memory KJ1 .26 ( + ) CD4 ( + ) T cells from wild-type mice were detected in the spleen , lungs and liver during 10 weeks after immunization ; however , Bcl6-deficient KJ1 .26 ( + ) CD4 ( + ) T cells were vanished completely in those organs 4 weeks after immunization .
	manualset3
238407	3	423434	15	NULL	NULL	0	NULL	spleen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term memory KJ1 .26 ( + ) CD4 ( + ) T cells from wild-type mice were detected in the spleen , lungs and liver during 10 weeks after immunization ; however , Bcl6-deficient KJ1 .26 ( + ) CD4 ( + ) T cells were vanished completely in those organs 4 weeks after immunization .
	manualset3
238408	4	423434	15	NULL	NULL	0	NULL	lungs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term memory KJ1 .26 ( + ) CD4 ( + ) T cells from wild-type mice were detected in the spleen , lungs and liver during 10 weeks after immunization ; however , Bcl6-deficient KJ1 .26 ( + ) CD4 ( + ) T cells were vanished completely in those organs 4 weeks after immunization .
	manualset3
238409	5	423434	15	NULL	NULL	0	NULL	 liver 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term memory KJ1 .26 ( + ) CD4 ( + ) T cells from wild-type mice were detected in the spleen , lungs and liver during 10 weeks after immunization ; however , Bcl6-deficient KJ1 .26 ( + ) CD4 ( + ) T cells were vanished completely in those organs 4 weeks after immunization .
	manualset3
238410	6	423434	15	NULL	NULL	0	NULL	10 weeks after immunization	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term memory KJ1 .26 ( + ) CD4 ( + ) T cells from wild-type mice were detected in the spleen , lungs and liver during 10 weeks after immunization ; however , Bcl6-deficient KJ1 .26 ( + ) CD4 ( + ) T cells were vanished completely in those organs 4 weeks after immunization .
	manualset3
238411	7	423434	15	NULL	NULL	0	NULL	Bcl6-deficient KJ1 .26 ( + ) CD4 ( + ) T cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Long-term memory KJ1 .26 ( + ) CD4 ( + ) T cells from wild-type mice were detected in the spleen , lungs and liver during 10 weeks after immunization ; however , Bcl6-deficient KJ1 .26 ( + ) CD4 ( + ) T cells were vanished completely in those organs 4 weeks after immunization .
	manualset3
238412	8	423434	15	NULL	NULL	NULL	NULL	organs 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Long-term memory KJ1 .26 ( + ) CD4 ( + ) T cells from wild-type mice were detected in the spleen , lungs and liver during 10 weeks after immunization ; however , Bcl6-deficient KJ1 .26 ( + ) CD4 ( + ) T cells were vanished completely in those organs 4 weeks after immunization .
	manualset3
258172	9	423434	15	NULL	NULL	NULL	NULL	4 weeks after immunization	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Long-term memory KJ1 .26 ( + ) CD4 ( + ) T cells from wild-type mice were detected in the spleen , lungs and liver during 10 weeks after immunization ; however , Bcl6-deficient KJ1 .26 ( + ) CD4 ( + ) T cells were vanished completely in those organs 4 weeks after immunization .
	manualset3
238416	1	423435	15	NULL	NULL	0	NULL	Orthopedic management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Orthopedic management of bone and joint tuberculosis in the tuberculosis advisory clinic ) .
	manualset3
238419	2	423435	15	NULL	NULL	0	NULL	 bone tuberculosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Orthopedic management of bone and joint tuberculosis in the tuberculosis advisory clinic ) .
	manualset3
238421	3	423435	15	NULL	NULL	0	NULL	joint tuberculosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Orthopedic management of bone and joint tuberculosis in the tuberculosis advisory clinic ) .
	manualset3
238423	4	423435	15	NULL	NULL	0	NULL	tuberculosis advisory clinic	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( Orthopedic management of bone and joint tuberculosis in the tuberculosis advisory clinic ) .
	manualset3
238436	1	423436	15	NULL	NULL	0	NULL	Thyroid-associated ophthalmopathy ( TAO )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Thyroid-associated ophthalmopathy ( TAO ) is most likely to be a T cell-mediated disease , in which cytokines released in the extraocular muscles activate fibroblasts , increasing glycosaminoglycan production .
	manualset3
238437	2	423436	15	NULL	NULL	0	NULL	T cell-mediated disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Thyroid-associated ophthalmopathy ( TAO ) is most likely to be a T cell-mediated disease , in which cytokines released in the extraocular muscles activate fibroblasts , increasing glycosaminoglycan production .
	manualset3
238438	3	423436	15	NULL	NULL	0	NULL	cytokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Thyroid-associated ophthalmopathy ( TAO ) is most likely to be a T cell-mediated disease , in which cytokines released in the extraocular muscles activate fibroblasts , increasing glycosaminoglycan production .
	manualset3
238440	4	423436	15	NULL	NULL	0	NULL	extraocular muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Thyroid-associated ophthalmopathy ( TAO ) is most likely to be a T cell-mediated disease , in which cytokines released in the extraocular muscles activate fibroblasts , increasing glycosaminoglycan production .
	manualset3
238442	5	423436	15	NULL	NULL	0	NULL	fibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Thyroid-associated ophthalmopathy ( TAO ) is most likely to be a T cell-mediated disease , in which cytokines released in the extraocular muscles activate fibroblasts , increasing glycosaminoglycan production .
	manualset3
238446	6	423436	15	NULL	NULL	0	NULL	glycosaminoglycan production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Thyroid-associated ophthalmopathy ( TAO ) is most likely to be a T cell-mediated disease , in which cytokines released in the extraocular muscles activate fibroblasts , increasing glycosaminoglycan production .
	manualset3
238453	1	423437	15	NULL	NULL	0	NULL	magnetic shock	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	When a magnetic shock but not stretch was given , a decrease in background EMG in the ipsilateral finger flexors occurred at a latency of 33 + / - 6.2 ms after the stimulus and with a duration of 25 + / - 8.5 ms. 3 .
	manualset3
238455	2	423437	15	NULL	NULL	0	NULL	stretch	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	When a magnetic shock but not stretch was given , a decrease in background EMG in the ipsilateral finger flexors occurred at a latency of 33 + / - 6.2 ms after the stimulus and with a duration of 25 + / - 8.5 ms. 3 .
	manualset3
238490	3	423437	15	NULL	NULL	0	NULL	decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	When a magnetic shock but not stretch was given , a decrease in background EMG in the ipsilateral finger flexors occurred at a latency of 33 + / - 6.2 ms after the stimulus and with a duration of 25 + / - 8.5 ms. 3 .
	manualset3
238491	4	423437	15	NULL	NULL	0	NULL	background EMG	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	When a magnetic shock but not stretch was given , a decrease in background EMG in the ipsilateral finger flexors occurred at a latency of 33 + / - 6.2 ms after the stimulus and with a duration of 25 + / - 8.5 ms. 3 .
	manualset3
238494	5	423437	15	NULL	NULL	0	NULL	ipsilateral finger flexors	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	When a magnetic shock but not stretch was given , a decrease in background EMG in the ipsilateral finger flexors occurred at a latency of 33 + / - 6.2 ms after the stimulus and with a duration of 25 + / - 8.5 ms. 3 .
	manualset3
238496	6	423437	15	NULL	NULL	NULL	NULL	latency	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When a magnetic shock but not stretch was given , a decrease in background EMG in the ipsilateral finger flexors occurred at a latency of 33 + / - 6.2 ms after the stimulus and with a duration of 25 + / - 8.5 ms. 3 .
	manualset3
238499	8	423437	15	NULL	NULL	NULL	NULL	stimulus	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When a magnetic shock but not stretch was given , a decrease in background EMG in the ipsilateral finger flexors occurred at a latency of 33 + / - 6.2 ms after the stimulus and with a duration of 25 + / - 8.5 ms. 3 .
	manualset3
238500	9	423437	15	NULL	NULL	NULL	NULL	duration	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When a magnetic shock but not stretch was given , a decrease in background EMG in the ipsilateral finger flexors occurred at a latency of 33 + / - 6.2 ms after the stimulus and with a duration of 25 + / - 8.5 ms. 3 .
	manualset3
258181	10	423437	15	NULL	NULL	NULL	NULL	25 + / - 8.5 ms. 3	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When a magnetic shock but not stretch was given , a decrease in background EMG in the ipsilateral finger flexors occurred at a latency of 33 + / - 6.2 ms after the stimulus and with a duration of 25 + / - 8.5 ms. 3 .
	manualset3
258668	7	423437	15	NULL	NULL	NULL	NULL	33 + / - 6.2 ms	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	When a magnetic shock but not stretch was given , a decrease in background EMG in the ipsilateral finger flexors occurred at a latency of 33 + / - 6.2 ms after the stimulus and with a duration of 25 + / - 8.5 ms. 3 .
	manualset3
238501	1	423438	15	NULL	NULL	0	NULL	Nutrition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nutrition as primary therapy in pediatric Crohn 's disease : fact or fantasy ?
	manualset3
238502	2	423438	15	NULL	NULL	0	NULL	primary therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Nutrition as primary therapy in pediatric Crohn 's disease : fact or fantasy ?
	manualset3
238503	3	423438	15	NULL	NULL	0	NULL	pediatric Crohn 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Nutrition as primary therapy in pediatric Crohn 's disease : fact or fantasy ?
	manualset3
238504	4	423438	15	NULL	NULL	0	NULL	fact	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nutrition as primary therapy in pediatric Crohn 's disease : fact or fantasy ?
	manualset3
238505	5	423438	15	NULL	NULL	0	NULL	fantasy	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Nutrition as primary therapy in pediatric Crohn 's disease : fact or fantasy ?
	manualset3
238510	1	423439	15	NULL	NULL	0	NULL	Surgical management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Surgical management of large fistula of the cecum or of the terminal segment of the ileum ) .
	manualset3
238513	2	423439	15	NULL	NULL	0	NULL	large fistula of the cecum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Surgical management of large fistula of the cecum or of the terminal segment of the ileum ) .
	manualset3
238515	3	423439	15	NULL	NULL	0	NULL	terminal segment of the ileum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Surgical management of large fistula of the cecum or of the terminal segment of the ileum ) .
	manualset3
238519	1	423440	15	NULL	NULL	0	NULL	Peritoneal drainage 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Peritoneal drainage has been reported as an initial resuscitative procedure for unstable infants who have complicated NEC .
	manualset3
238520	2	423440	15	NULL	NULL	0	NULL	initial resuscitative procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Peritoneal drainage has been reported as an initial resuscitative procedure for unstable infants who have complicated NEC .
	manualset3
238522	3	423440	15	NULL	NULL	0	NULL	infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Peritoneal drainage has been reported as an initial resuscitative procedure for unstable infants who have complicated NEC .
	manualset3
238526	4	423440	15	NULL	NULL	0	NULL	NEC	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Peritoneal drainage has been reported as an initial resuscitative procedure for unstable infants who have complicated NEC .
	manualset3
238533	1	423441	15	NULL	NULL	0	NULL	data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Taken together , these data suggest that the CAIII-promoted invasive ability of HCC cells may probably be mediated through , at least in part , the FAK signaling pathway via intracellular and/or extracellular acidification .
	manualset3
238537	2	423441	15	NULL	NULL	0	NULL	CAIII-promoted invasive ability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Taken together , these data suggest that the CAIII-promoted invasive ability of HCC cells may probably be mediated through , at least in part , the FAK signaling pathway via intracellular and/or extracellular acidification .
	manualset3
238539	3	423441	15	NULL	NULL	0	NULL	HCC cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Taken together , these data suggest that the CAIII-promoted invasive ability of HCC cells may probably be mediated through , at least in part , the FAK signaling pathway via intracellular and/or extracellular acidification .
	manualset3
238548	5	423441	15	NULL	NULL	NULL	NULL	intracellular acidification	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Taken together , these data suggest that the CAIII-promoted invasive ability of HCC cells may probably be mediated through , at least in part , the FAK signaling pathway via intracellular and/or extracellular acidification .
	manualset3
238549	6	423441	15	NULL	NULL	NULL	NULL	extracellular acidification	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Taken together , these data suggest that the CAIII-promoted invasive ability of HCC cells may probably be mediated through , at least in part , the FAK signaling pathway via intracellular and/or extracellular acidification .
	manualset3
258188	4	423441	15	NULL	NULL	NULL	NULL	FAK signaling pathway	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Taken together , these data suggest that the CAIII-promoted invasive ability of HCC cells may probably be mediated through , at least in part , the FAK signaling pathway via intracellular and/or extracellular acidification .
	manualset3
238564	1	423442	15	NULL	NULL	NULL	NULL	reactions of Na ( 2 ) 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The reactions of Na ( 2 ) with a series of atmospheric constituents were studied using a fast flow tube with detection of Na ( 2 ) by laser induced fluorescence at 656.2 nm ( Na ( 2 ) ( A ( 1 ) Sigma ( + ) ( u ) - X ( 1 ) Sigma ( + ) ( g ) ) ) .
	manualset3
238583	2	423442	15	NULL	NULL	0	NULL	series	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The reactions of Na ( 2 ) with a series of atmospheric constituents were studied using a fast flow tube with detection of Na ( 2 ) by laser induced fluorescence at 656.2 nm ( Na ( 2 ) ( A ( 1 ) Sigma ( + ) ( u ) - X ( 1 ) Sigma ( + ) ( g ) ) ) .
	manualset3
238588	3	423442	15	NULL	NULL	0	NULL	atmospheric constituents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The reactions of Na ( 2 ) with a series of atmospheric constituents were studied using a fast flow tube with detection of Na ( 2 ) by laser induced fluorescence at 656.2 nm ( Na ( 2 ) ( A ( 1 ) Sigma ( + ) ( u ) - X ( 1 ) Sigma ( + ) ( g ) ) ) .
	manualset3
238589	4	423442	15	NULL	NULL	0	NULL	fast flow tube	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	The reactions of Na ( 2 ) with a series of atmospheric constituents were studied using a fast flow tube with detection of Na ( 2 ) by laser induced fluorescence at 656.2 nm ( Na ( 2 ) ( A ( 1 ) Sigma ( + ) ( u ) - X ( 1 ) Sigma ( + ) ( g ) ) ) .
	manualset3
238590	5	423442	15	NULL	NULL	0	NULL	detection of Na ( 2 )	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The reactions of Na ( 2 ) with a series of atmospheric constituents were studied using a fast flow tube with detection of Na ( 2 ) by laser induced fluorescence at 656.2 nm ( Na ( 2 ) ( A ( 1 ) Sigma ( + ) ( u ) - X ( 1 ) Sigma ( + ) ( g ) ) ) .
	manualset3
238647	6	423442	15	NULL	NULL	0	NULL	laser induced fluorescence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The reactions of Na ( 2 ) with a series of atmospheric constituents were studied using a fast flow tube with detection of Na ( 2 ) by laser induced fluorescence at 656.2 nm ( Na ( 2 ) ( A ( 1 ) Sigma ( + ) ( u ) - X ( 1 ) Sigma ( + ) ( g ) ) ) .
	manualset3
238648	7	423442	15	NULL	NULL	0	NULL	656.2 nm ( Na ( 2 ) ( A ( 1 ) Sigma ( + ) ( u ) - X ( 1 ) Sigma ( + ) ( g ) ) )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The reactions of Na ( 2 ) with a series of atmospheric constituents were studied using a fast flow tube with detection of Na ( 2 ) by laser induced fluorescence at 656.2 nm ( Na ( 2 ) ( A ( 1 ) Sigma ( + ) ( u ) - X ( 1 ) Sigma ( + ) ( g ) ) ) .
	manualset3
238649	1	423443	15	NULL	NULL	0	NULL	Liver biopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver biopsy is essential for the accurate assessment of patients with non-HFE hemochromatosis and in patients who have dual pathology .
	manualset3
238650	2	423443	15	NULL	NULL	0	NULL	accurate assessment of patients	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver biopsy is essential for the accurate assessment of patients with non-HFE hemochromatosis and in patients who have dual pathology .
	manualset3
238651	3	423443	15	NULL	NULL	0	NULL	non-HFE hemochromatosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver biopsy is essential for the accurate assessment of patients with non-HFE hemochromatosis and in patients who have dual pathology .
	manualset3
238652	4	423443	15	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver biopsy is essential for the accurate assessment of patients with non-HFE hemochromatosis and in patients who have dual pathology .
	manualset3
238653	5	423443	15	NULL	NULL	0	NULL	dual pathology 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Liver biopsy is essential for the accurate assessment of patients with non-HFE hemochromatosis and in patients who have dual pathology .
	manualset3
238654	1	423444	15	NULL	NULL	0	NULL	Ecological relevance	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Ecological relevance of chemically induced endocrine disruption in wildlife .
	manualset3
238655	2	423444	15	NULL	NULL	0	NULL	chemically induced endocrine disruption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ecological relevance of chemically induced endocrine disruption in wildlife .
	manualset3
238656	3	423444	15	NULL	NULL	0	NULL	wildlife	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ecological relevance of chemically induced endocrine disruption in wildlife .
	manualset3
238657	1	423445	15	NULL	NULL	0	NULL	pharmacokinetic parameters	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Individual pharmacokinetic parameters of DHPG were determined and were markedly altered .
	manualset3
238658	2	423445	15	NULL	NULL	0	NULL	DHPG	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Individual pharmacokinetic parameters of DHPG were determined and were markedly altered .
	manualset3
238659	1	423446	15	NULL	NULL	0	NULL	gas chromatography-mass spectrometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	We utilized gas chromatography-mass spectrometry to study the transfer of 15N from ( 2-15N ) glutamine , ( 15N ) leucine , ( 15N ) alanine , or 15NH4Cl to ( 15N ) glutamate and ( 15N ) aspartate in cultured cerebrocortical GABA-ergic neurons from the mouse .
	manualset3
238660	2	423446	15	NULL	NULL	0	NULL	transfer	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	We utilized gas chromatography-mass spectrometry to study the transfer of 15N from ( 2-15N ) glutamine , ( 15N ) leucine , ( 15N ) alanine , or 15NH4Cl to ( 15N ) glutamate and ( 15N ) aspartate in cultured cerebrocortical GABA-ergic neurons from the mouse .
	manualset3
238661	3	423446	15	NULL	NULL	0	NULL	15N	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	We utilized gas chromatography-mass spectrometry to study the transfer of 15N from ( 2-15N ) glutamine , ( 15N ) leucine , ( 15N ) alanine , or 15NH4Cl to ( 15N ) glutamate and ( 15N ) aspartate in cultured cerebrocortical GABA-ergic neurons from the mouse .
	manualset3
238662	4	423446	15	NULL	NULL	0	NULL	( 2-15N ) glutamine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	We utilized gas chromatography-mass spectrometry to study the transfer of 15N from ( 2-15N ) glutamine , ( 15N ) leucine , ( 15N ) alanine , or 15NH4Cl to ( 15N ) glutamate and ( 15N ) aspartate in cultured cerebrocortical GABA-ergic neurons from the mouse .
	manualset3
238663	5	423446	15	NULL	NULL	0	NULL	( 15N ) leucine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	We utilized gas chromatography-mass spectrometry to study the transfer of 15N from ( 2-15N ) glutamine , ( 15N ) leucine , ( 15N ) alanine , or 15NH4Cl to ( 15N ) glutamate and ( 15N ) aspartate in cultured cerebrocortical GABA-ergic neurons from the mouse .
	manualset3
238664	6	423446	15	NULL	NULL	0	NULL	( 15N ) alanine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	We utilized gas chromatography-mass spectrometry to study the transfer of 15N from ( 2-15N ) glutamine , ( 15N ) leucine , ( 15N ) alanine , or 15NH4Cl to ( 15N ) glutamate and ( 15N ) aspartate in cultured cerebrocortical GABA-ergic neurons from the mouse .
	manualset3
238665	7	423446	15	NULL	NULL	0	NULL	15NH4Cl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	We utilized gas chromatography-mass spectrometry to study the transfer of 15N from ( 2-15N ) glutamine , ( 15N ) leucine , ( 15N ) alanine , or 15NH4Cl to ( 15N ) glutamate and ( 15N ) aspartate in cultured cerebrocortical GABA-ergic neurons from the mouse .
	manualset3
238666	8	423446	15	NULL	NULL	0	NULL	( 15N ) glutamate	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	We utilized gas chromatography-mass spectrometry to study the transfer of 15N from ( 2-15N ) glutamine , ( 15N ) leucine , ( 15N ) alanine , or 15NH4Cl to ( 15N ) glutamate and ( 15N ) aspartate in cultured cerebrocortical GABA-ergic neurons from the mouse .
	manualset3
238667	9	423446	15	NULL	NULL	0	NULL	( 15N ) aspartate	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	We utilized gas chromatography-mass spectrometry to study the transfer of 15N from ( 2-15N ) glutamine , ( 15N ) leucine , ( 15N ) alanine , or 15NH4Cl to ( 15N ) glutamate and ( 15N ) aspartate in cultured cerebrocortical GABA-ergic neurons from the mouse .
	manualset3
238668	10	423446	15	NULL	NULL	0	NULL	cerebrocortical GABA-ergic neurons	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	We utilized gas chromatography-mass spectrometry to study the transfer of 15N from ( 2-15N ) glutamine , ( 15N ) leucine , ( 15N ) alanine , or 15NH4Cl to ( 15N ) glutamate and ( 15N ) aspartate in cultured cerebrocortical GABA-ergic neurons from the mouse .
	manualset3
238669	11	423446	15	NULL	NULL	0	NULL	mouse	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	We utilized gas chromatography-mass spectrometry to study the transfer of 15N from ( 2-15N ) glutamine , ( 15N ) leucine , ( 15N ) alanine , or 15NH4Cl to ( 15N ) glutamate and ( 15N ) aspartate in cultured cerebrocortical GABA-ergic neurons from the mouse .
	manualset3
238670	1	423447	15	NULL	NULL	0	NULL	host	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	As host for infective agents , as modulator of specific immune activity and as ultimate mediator of the host response , the macrophage plays a virtuoso 's role in the host-parasite drama .
	manualset3
238671	2	423447	15	NULL	NULL	NULL	NULL	infective agents	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As host for infective agents , as modulator of specific immune activity and as ultimate mediator of the host response , the macrophage plays a virtuoso 's role in the host-parasite drama .
	manualset3
238672	3	423447	15	NULL	NULL	NULL	NULL	modulator	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As host for infective agents , as modulator of specific immune activity and as ultimate mediator of the host response , the macrophage plays a virtuoso 's role in the host-parasite drama .
	manualset3
238673	4	423447	15	NULL	NULL	0	NULL	specific immune activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As host for infective agents , as modulator of specific immune activity and as ultimate mediator of the host response , the macrophage plays a virtuoso 's role in the host-parasite drama .
	manualset3
238674	5	423447	15	NULL	NULL	0	NULL	mediator	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As host for infective agents , as modulator of specific immune activity and as ultimate mediator of the host response , the macrophage plays a virtuoso 's role in the host-parasite drama .
	manualset3
238675	6	423447	15	NULL	NULL	0	NULL	host response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As host for infective agents , as modulator of specific immune activity and as ultimate mediator of the host response , the macrophage plays a virtuoso 's role in the host-parasite drama .
	manualset3
238676	7	423447	15	NULL	NULL	0	NULL	macrophage 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	As host for infective agents , as modulator of specific immune activity and as ultimate mediator of the host response , the macrophage plays a virtuoso 's role in the host-parasite drama .
	manualset3
238677	8	423447	15	NULL	NULL	NULL	NULL	virtuoso 's role	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As host for infective agents , as modulator of specific immune activity and as ultimate mediator of the host response , the macrophage plays a virtuoso 's role in the host-parasite drama .
	manualset3
238678	9	423447	15	NULL	NULL	0	NULL	host-parasite drama	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As host for infective agents , as modulator of specific immune activity and as ultimate mediator of the host response , the macrophage plays a virtuoso 's role in the host-parasite drama .
	manualset3
238683	1	423448	15	NULL	NULL	NULL	NULL	Semiconductor theory 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Semiconductor theory of ion transport in thin lipid membranes .
	manualset3
238684	3	423448	15	NULL	NULL	NULL	NULL	thin lipid membranes	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Semiconductor theory of ion transport in thin lipid membranes .
	manualset3
258226	2	423448	15	NULL	NULL	NULL	NULL	ion transport 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Semiconductor theory of ion transport in thin lipid membranes .
	manualset3
238685	1	423449	15	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was carried out in several groups of male Wistar rats weighing 300 gm and fed for 60 , 104 , 195 , 250 , and 336 hours with a choline-deficient diet supplemented with ethionine ( CDE ) .
	manualset3
238686	2	423449	15	NULL	NULL	0	NULL	several groups	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was carried out in several groups of male Wistar rats weighing 300 gm and fed for 60 , 104 , 195 , 250 , and 336 hours with a choline-deficient diet supplemented with ethionine ( CDE ) .
	manualset3
238687	3	423449	15	NULL	NULL	0	NULL	male Wistar rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was carried out in several groups of male Wistar rats weighing 300 gm and fed for 60 , 104 , 195 , 250 , and 336 hours with a choline-deficient diet supplemented with ethionine ( CDE ) .
	manualset3
238688	4	423449	15	NULL	NULL	0	NULL	 300 gm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was carried out in several groups of male Wistar rats weighing 300 gm and fed for 60 , 104 , 195 , 250 , and 336 hours with a choline-deficient diet supplemented with ethionine ( CDE ) .
	manualset3
238689	5	423449	15	NULL	NULL	0	NULL	60 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was carried out in several groups of male Wistar rats weighing 300 gm and fed for 60 , 104 , 195 , 250 , and 336 hours with a choline-deficient diet supplemented with ethionine ( CDE ) .
	manualset3
238691	6	423449	15	NULL	NULL	0	NULL	104 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was carried out in several groups of male Wistar rats weighing 300 gm and fed for 60 , 104 , 195 , 250 , and 336 hours with a choline-deficient diet supplemented with ethionine ( CDE ) .
	manualset3
238693	7	423449	15	NULL	NULL	0	NULL	195 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was carried out in several groups of male Wistar rats weighing 300 gm and fed for 60 , 104 , 195 , 250 , and 336 hours with a choline-deficient diet supplemented with ethionine ( CDE ) .
	manualset3
238696	8	423449	15	NULL	NULL	0	NULL	250 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was carried out in several groups of male Wistar rats weighing 300 gm and fed for 60 , 104 , 195 , 250 , and 336 hours with a choline-deficient diet supplemented with ethionine ( CDE ) .
	manualset3
238697	9	423449	15	NULL	NULL	0	NULL	336 hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was carried out in several groups of male Wistar rats weighing 300 gm and fed for 60 , 104 , 195 , 250 , and 336 hours with a choline-deficient diet supplemented with ethionine ( CDE ) .
	manualset3
238700	10	423449	15	NULL	NULL	0	NULL	choline-deficient diet	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was carried out in several groups of male Wistar rats weighing 300 gm and fed for 60 , 104 , 195 , 250 , and 336 hours with a choline-deficient diet supplemented with ethionine ( CDE ) .
	manualset3
238702	11	423449	15	NULL	NULL	0	NULL	ethionine ( CDE )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	The study was carried out in several groups of male Wistar rats weighing 300 gm and fed for 60 , 104 , 195 , 250 , and 336 hours with a choline-deficient diet supplemented with ethionine ( CDE ) .
	manualset3
238706	1	423450	15	NULL	NULL	0	NULL	Neurobehaviors	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurobehaviors and psychotic symptoms in Alzheimer 's disease .
	manualset3
238707	2	423450	15	NULL	NULL	0	NULL	psychotic symptoms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurobehaviors and psychotic symptoms in Alzheimer 's disease .
	manualset3
238708	3	423450	15	NULL	NULL	0	NULL	Alzheimer 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Neurobehaviors and psychotic symptoms in Alzheimer 's disease .
	manualset3
239118	1	423451	15	NULL	NULL	0	NULL	Pre - ganglionic nerve fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre - and post-ganglionic nerve fibers of the pterygopalatine ganglion and their allocation to the eyeball of rats .
	manualset3
239120	2	423451	15	NULL	NULL	0	NULL	post-ganglionic nerve fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre - and post-ganglionic nerve fibers of the pterygopalatine ganglion and their allocation to the eyeball of rats .
	manualset3
239127	3	423451	15	NULL	NULL	0	NULL	pterygopalatine ganglion	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre - and post-ganglionic nerve fibers of the pterygopalatine ganglion and their allocation to the eyeball of rats .
	manualset3
239128	4	423451	15	NULL	NULL	0	NULL	 allocation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre - and post-ganglionic nerve fibers of the pterygopalatine ganglion and their allocation to the eyeball of rats .
	manualset3
239129	5	423451	15	NULL	NULL	0	NULL	 eyeball 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre - and post-ganglionic nerve fibers of the pterygopalatine ganglion and their allocation to the eyeball of rats .
	manualset3
239130	6	423451	15	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Pre - and post-ganglionic nerve fibers of the pterygopalatine ganglion and their allocation to the eyeball of rats .
	manualset3
239131	1	423452	15	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	The present studies assessed the role of G ( zalpha ) and G ( oalpha ) in spinal alpha ( 2 ) adrenergic receptor agonist-induced antinociception , as well as in antinociceptive synergism between spinal morphine and clonidine .
	manualset3
239132	2	423452	15	NULL	NULL	NULL	NULL	role of G ( zalpha )	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present studies assessed the role of G ( zalpha ) and G ( oalpha ) in spinal alpha ( 2 ) adrenergic receptor agonist-induced antinociception , as well as in antinociceptive synergism between spinal morphine and clonidine .
	manualset3
239133	3	423452	15	NULL	NULL	0	NULL	role of G ( oalpha )	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	The present studies assessed the role of G ( zalpha ) and G ( oalpha ) in spinal alpha ( 2 ) adrenergic receptor agonist-induced antinociception , as well as in antinociceptive synergism between spinal morphine and clonidine .
	manualset3
239134	4	423452	15	NULL	NULL	NULL	NULL	spinal alpha ( 2 ) adrenergic receptor agonist-induced antinociception	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	The present studies assessed the role of G ( zalpha ) and G ( oalpha ) in spinal alpha ( 2 ) adrenergic receptor agonist-induced antinociception , as well as in antinociceptive synergism between spinal morphine and clonidine .
	manualset3
239135	5	423452	15	NULL	NULL	0	NULL	antinociceptive synergism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	The present studies assessed the role of G ( zalpha ) and G ( oalpha ) in spinal alpha ( 2 ) adrenergic receptor agonist-induced antinociception , as well as in antinociceptive synergism between spinal morphine and clonidine .
	manualset3
239138	6	423452	15	NULL	NULL	0	NULL	morphine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The present studies assessed the role of G ( zalpha ) and G ( oalpha ) in spinal alpha ( 2 ) adrenergic receptor agonist-induced antinociception , as well as in antinociceptive synergism between spinal morphine and clonidine .
	manualset3
239140	7	423452	15	NULL	NULL	0	NULL	clonidine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	The present studies assessed the role of G ( zalpha ) and G ( oalpha ) in spinal alpha ( 2 ) adrenergic receptor agonist-induced antinociception , as well as in antinociceptive synergism between spinal morphine and clonidine .
	manualset3
239149	1	423453	15	NULL	NULL	NULL	NULL	Anatomical specificity 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Anatomical specificity within rat striatum for the dopaminergic modulation of DRL responding and activity .
	manualset3
239150	2	423453	15	NULL	NULL	0	NULL	rat striatum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomical specificity within rat striatum for the dopaminergic modulation of DRL responding and activity .
	manualset3
239151	3	423453	15	NULL	NULL	0	NULL	dopaminergic modulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomical specificity within rat striatum for the dopaminergic modulation of DRL responding and activity .
	manualset3
239154	4	423453	15	NULL	NULL	0	NULL	DRL responding	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomical specificity within rat striatum for the dopaminergic modulation of DRL responding and activity .
	manualset3
239155	5	423453	15	NULL	NULL	NULL	NULL	activity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Anatomical specificity within rat striatum for the dopaminergic modulation of DRL responding and activity .
	manualset3
239158	1	423454	15	NULL	NULL	0	NULL	Anatomical tracer studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomical tracer studies reveal projections from the vlPOA and MnPN to multiple arousal-regulatory systems in the posterior and lateral hypothalamus and the rostral brainstem .
	manualset3
239168	2	423454	15	NULL	NULL	0	NULL	projections	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomical tracer studies reveal projections from the vlPOA and MnPN to multiple arousal-regulatory systems in the posterior and lateral hypothalamus and the rostral brainstem .
	manualset3
239169	3	423454	15	NULL	NULL	0	NULL	vlPOA	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomical tracer studies reveal projections from the vlPOA and MnPN to multiple arousal-regulatory systems in the posterior and lateral hypothalamus and the rostral brainstem .
	manualset3
239170	4	423454	15	NULL	NULL	0	NULL	MnPN	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomical tracer studies reveal projections from the vlPOA and MnPN to multiple arousal-regulatory systems in the posterior and lateral hypothalamus and the rostral brainstem .
	manualset3
239172	5	423454	15	NULL	NULL	0	NULL	multiple arousal-regulatory systems	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomical tracer studies reveal projections from the vlPOA and MnPN to multiple arousal-regulatory systems in the posterior and lateral hypothalamus and the rostral brainstem .
	manualset3
239175	6	423454	15	NULL	NULL	0	NULL	posterior hypothalamus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomical tracer studies reveal projections from the vlPOA and MnPN to multiple arousal-regulatory systems in the posterior and lateral hypothalamus and the rostral brainstem .
	manualset3
239177	7	423454	15	NULL	NULL	0	NULL	lateral hypothalamus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomical tracer studies reveal projections from the vlPOA and MnPN to multiple arousal-regulatory systems in the posterior and lateral hypothalamus and the rostral brainstem .
	manualset3
239179	8	423454	15	NULL	NULL	0	NULL	rostral brainstem	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomical tracer studies reveal projections from the vlPOA and MnPN to multiple arousal-regulatory systems in the posterior and lateral hypothalamus and the rostral brainstem .
	manualset3
239185	1	423455	15	NULL	NULL	0	NULL	Drug prevention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Drug prevention and therapy of ventricular tachycardia ) .
	manualset3
239187	2	423455	15	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Drug prevention and therapy of ventricular tachycardia ) .
	manualset3
239190	3	423455	15	NULL	NULL	0	NULL	ventricular tachycardia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Drug prevention and therapy of ventricular tachycardia ) .
	manualset3
239192	1	423456	15	NULL	NULL	0	NULL	Anatomo-biological correlations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomo-biological correlations for pulmonary transplantation ) .
	manualset3
239193	2	423456	15	NULL	NULL	0	NULL	pulmonary transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomo-biological correlations for pulmonary transplantation ) .
	manualset3
239196	1	423457	15	NULL	NULL	0	NULL	Anatomy	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomy , nomenclature , first clinical observations : In ancient Greece and Rome and in the Middle Ages the posterior opening of the nasal passage was known ( Greek `` choane '' = funnel ) as an atomical structure , and it was also known that chronic nasal catarrh is common in children , but it was not realized that this was associated with special pathological alterations .
	manualset3
239198	2	423457	15	NULL	NULL	0	NULL	nomenclature	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomy , nomenclature , first clinical observations : In ancient Greece and Rome and in the Middle Ages the posterior opening of the nasal passage was known ( Greek `` choane '' = funnel ) as an atomical structure , and it was also known that chronic nasal catarrh is common in children , but it was not realized that this was associated with special pathological alterations .
	manualset3
239199	3	423457	15	NULL	NULL	0	NULL	clinical observations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomy , nomenclature , first clinical observations : In ancient Greece and Rome and in the Middle Ages the posterior opening of the nasal passage was known ( Greek `` choane '' = funnel ) as an atomical structure , and it was also known that chronic nasal catarrh is common in children , but it was not realized that this was associated with special pathological alterations .
	manualset3
239203	4	423457	15	NULL	NULL	0	NULL	Greece	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomy , nomenclature , first clinical observations : In ancient Greece and Rome and in the Middle Ages the posterior opening of the nasal passage was known ( Greek `` choane '' = funnel ) as an atomical structure , and it was also known that chronic nasal catarrh is common in children , but it was not realized that this was associated with special pathological alterations .
	manualset3
239204	5	423457	15	NULL	NULL	0	NULL	Rome	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomy , nomenclature , first clinical observations : In ancient Greece and Rome and in the Middle Ages the posterior opening of the nasal passage was known ( Greek `` choane '' = funnel ) as an atomical structure , and it was also known that chronic nasal catarrh is common in children , but it was not realized that this was associated with special pathological alterations .
	manualset3
239207	6	423457	15	NULL	NULL	0	NULL	Middle Ages	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomy , nomenclature , first clinical observations : In ancient Greece and Rome and in the Middle Ages the posterior opening of the nasal passage was known ( Greek `` choane '' = funnel ) as an atomical structure , and it was also known that chronic nasal catarrh is common in children , but it was not realized that this was associated with special pathological alterations .
	manualset3
239213	7	423457	15	NULL	NULL	NULL	NULL	posterior opening of the nasal passage	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Anatomy , nomenclature , first clinical observations : In ancient Greece and Rome and in the Middle Ages the posterior opening of the nasal passage was known ( Greek `` choane '' = funnel ) as an atomical structure , and it was also known that chronic nasal catarrh is common in children , but it was not realized that this was associated with special pathological alterations .
	manualset3
239217	8	423457	15	NULL	NULL	0	NULL	Greek	Language												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomy , nomenclature , first clinical observations : In ancient Greece and Rome and in the Middle Ages the posterior opening of the nasal passage was known ( Greek `` choane '' = funnel ) as an atomical structure , and it was also known that chronic nasal catarrh is common in children , but it was not realized that this was associated with special pathological alterations .
	manualset3
239218	9	423457	15	NULL	NULL	0	NULL	choane	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomy , nomenclature , first clinical observations : In ancient Greece and Rome and in the Middle Ages the posterior opening of the nasal passage was known ( Greek `` choane '' = funnel ) as an atomical structure , and it was also known that chronic nasal catarrh is common in children , but it was not realized that this was associated with special pathological alterations .
	manualset3
239219	10	423457	15	NULL	NULL	0	NULL	funnel	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomy , nomenclature , first clinical observations : In ancient Greece and Rome and in the Middle Ages the posterior opening of the nasal passage was known ( Greek `` choane '' = funnel ) as an atomical structure , and it was also known that chronic nasal catarrh is common in children , but it was not realized that this was associated with special pathological alterations .
	manualset3
239220	11	423457	15	NULL	NULL	0	NULL	atomical structure	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomy , nomenclature , first clinical observations : In ancient Greece and Rome and in the Middle Ages the posterior opening of the nasal passage was known ( Greek `` choane '' = funnel ) as an atomical structure , and it was also known that chronic nasal catarrh is common in children , but it was not realized that this was associated with special pathological alterations .
	manualset3
239221	12	423457	15	NULL	NULL	0	NULL	chronic nasal catarrh 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomy , nomenclature , first clinical observations : In ancient Greece and Rome and in the Middle Ages the posterior opening of the nasal passage was known ( Greek `` choane '' = funnel ) as an atomical structure , and it was also known that chronic nasal catarrh is common in children , but it was not realized that this was associated with special pathological alterations .
	manualset3
239222	13	423457	15	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomy , nomenclature , first clinical observations : In ancient Greece and Rome and in the Middle Ages the posterior opening of the nasal passage was known ( Greek `` choane '' = funnel ) as an atomical structure , and it was also known that chronic nasal catarrh is common in children , but it was not realized that this was associated with special pathological alterations .
	manualset3
239223	14	423457	15	NULL	NULL	0	NULL	pathological alterations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Anatomy , nomenclature , first clinical observations : In ancient Greece and Rome and in the Middle Ages the posterior opening of the nasal passage was known ( Greek `` choane '' = funnel ) as an atomical structure , and it was also known that chronic nasal catarrh is common in children , but it was not realized that this was associated with special pathological alterations .
	manualset3
239232	1	423458	15	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Ancestral ability to use dry beans has been lost in the chinensis clade but acquired again in C. chinensis .
	manualset3
239234	2	423458	15	NULL	NULL	0	NULL	dry beans	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Ancestral ability to use dry beans has been lost in the chinensis clade but acquired again in C. chinensis .
	manualset3
239235	3	423458	15	NULL	NULL	0	NULL	chinensis clade	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ancestral ability to use dry beans has been lost in the chinensis clade but acquired again in C. chinensis .
	manualset3
239236	4	423458	15	NULL	NULL	0	NULL	C. chinensis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ancestral ability to use dry beans has been lost in the chinensis clade but acquired again in C. chinensis .
	manualset3
239237	1	423459	15	NULL	NULL	0	NULL	Pbx-Hox signatures 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ancient Pbx-Hox signatures define hundreds of vertebrate developmental enhancers .
	manualset3
239238	2	423459	15	NULL	NULL	0	NULL	hundreds 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Ancient Pbx-Hox signatures define hundreds of vertebrate developmental enhancers .
	manualset3
239239	3	423459	15	NULL	NULL	0	NULL	vertebrate developmental enhancers	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Ancient Pbx-Hox signatures define hundreds of vertebrate developmental enhancers .
	manualset3
239240	1	423460	15	NULL	NULL	0	NULL	members	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	And , with the members of the nation 's largest medical association auxiliary and their spouses behind Mrs. Haisten , Texas will see red -- red ribbons -- Oct 22-29 .
	manualset3
239241	2	423460	15	NULL	NULL	0	NULL	nation 's largest medical association auxiliary	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	And , with the members of the nation 's largest medical association auxiliary and their spouses behind Mrs. Haisten , Texas will see red -- red ribbons -- Oct 22-29 .
	manualset3
239242	3	423460	15	NULL	NULL	0	NULL	spouses	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	And , with the members of the nation 's largest medical association auxiliary and their spouses behind Mrs. Haisten , Texas will see red -- red ribbons -- Oct 22-29 .
	manualset3
239243	4	423460	15	NULL	NULL	0	NULL	Mrs. Haisten	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	And , with the members of the nation 's largest medical association auxiliary and their spouses behind Mrs. Haisten , Texas will see red -- red ribbons -- Oct 22-29 .
	manualset3
239244	5	423460	15	NULL	NULL	0	NULL	Texas	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	And , with the members of the nation 's largest medical association auxiliary and their spouses behind Mrs. Haisten , Texas will see red -- red ribbons -- Oct 22-29 .
	manualset3
239245	6	423460	15	NULL	NULL	0	NULL	ribbons	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	And , with the members of the nation 's largest medical association auxiliary and their spouses behind Mrs. Haisten , Texas will see red -- red ribbons -- Oct 22-29 .
	manualset3
239246	7	423460	15	NULL	NULL	0	NULL	Oct 22-29	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	And , with the members of the nation 's largest medical association auxiliary and their spouses behind Mrs. Haisten , Texas will see red -- red ribbons -- Oct 22-29 .
	manualset3
239247	1	423461	15	NULL	NULL	0	NULL	fact	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	And thus this fact should not change the actual diagnosis and prognostic implications .
	manualset3
239248	2	423461	15	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	And thus this fact should not change the actual diagnosis and prognostic implications .
	manualset3
239249	3	423461	15	NULL	NULL	0	NULL	prognostic implications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	And thus this fact should not change the actual diagnosis and prognostic implications .
	manualset3
239250	1	423462	15	NULL	NULL	0	NULL	Androgen-independent growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Androgen-independent growth is induced by neuropeptides in human prostate cancer cell lines .
	manualset3
239251	2	423462	15	NULL	NULL	0	NULL	neuropeptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Androgen-independent growth is induced by neuropeptides in human prostate cancer cell lines .
	manualset3
239252	3	423462	15	NULL	NULL	0	NULL	human prostate cancer cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Androgen-independent growth is induced by neuropeptides in human prostate cancer cell lines .
	manualset3
239253	1	423463	15	NULL	NULL	0	NULL	Androgen signaling	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Androgen signaling maintains expression of dkk1b and igfbp2a , which encode secreted inhibitors of Wnt and Igf signaling , respectively .
	manualset3
239254	2	423463	15	NULL	NULL	0	NULL	expression of dkk1b	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Androgen signaling maintains expression of dkk1b and igfbp2a , which encode secreted inhibitors of Wnt and Igf signaling , respectively .
	manualset3
239255	3	423463	15	NULL	NULL	0	NULL	expression of igfbp2a	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Androgen signaling maintains expression of dkk1b and igfbp2a , which encode secreted inhibitors of Wnt and Igf signaling , respectively .
	manualset3
239256	4	423463	15	NULL	NULL	0	NULL	inhibitors of Wnt signaling	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Androgen signaling maintains expression of dkk1b and igfbp2a , which encode secreted inhibitors of Wnt and Igf signaling , respectively .
	manualset3
239257	5	423463	15	NULL	NULL	0	NULL	 inhibitors of Igf signaling	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Androgen signaling maintains expression of dkk1b and igfbp2a , which encode secreted inhibitors of Wnt and Igf signaling , respectively .
	manualset3
239258	1	423464	15	NULL	NULL	0	NULL	Dynamic control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Dynamic control over venous return ) .
	manualset3
239259	2	423464	15	NULL	NULL	0	NULL	venous return	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Dynamic control over venous return ) .
	manualset3
239260	1	423465	15	NULL	NULL	NULL	NULL	Androstanolone	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Androstanolone represented about 2/3 , testosterone 1/10 , and the two androstanediols together 1/10 of the total radioactivity .
	manualset3
239261	2	423465	15	NULL	NULL	0	NULL	2/3	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Androstanolone represented about 2/3 , testosterone 1/10 , and the two androstanediols together 1/10 of the total radioactivity .
	manualset3
239262	3	423465	15	NULL	NULL	NULL	NULL	testosterone	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Androstanolone represented about 2/3 , testosterone 1/10 , and the two androstanediols together 1/10 of the total radioactivity .
	manualset3
239263	4	423465	15	NULL	NULL	0	NULL	1/10	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Androstanolone represented about 2/3 , testosterone 1/10 , and the two androstanediols together 1/10 of the total radioactivity .
	manualset3
239264	5	423465	15	NULL	NULL	NULL	NULL	two androstanediols	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Androstanolone represented about 2/3 , testosterone 1/10 , and the two androstanediols together 1/10 of the total radioactivity .
	manualset3
239265	6	423465	15	NULL	NULL	NULL	NULL	1/10 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Androstanolone represented about 2/3 , testosterone 1/10 , and the two androstanediols together 1/10 of the total radioactivity .
	manualset3
258244	7	423465	15	NULL	NULL	NULL	NULL	total radioactivity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Androstanolone represented about 2/3 , testosterone 1/10 , and the two androstanediols together 1/10 of the total radioactivity .
	manualset3
239266	1	423466	15	NULL	NULL	0	NULL	Anemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Anemia is common in chronic kidney disease ( CKD ) .
	manualset3
239267	2	423466	15	NULL	NULL	0	NULL	chronic kidney disease ( CKD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Anemia is common in chronic kidney disease ( CKD ) .
	manualset3
239268	1	423467	15	NULL	NULL	NULL	NULL	Anesthetic propofol 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Anesthetic propofol attenuates the isoflurane-induced caspase-3 activation and a oligomerization .
	manualset3
239269	2	423467	15	NULL	NULL	0	NULL	isoflurane-induced caspase-3 activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Anesthetic propofol attenuates the isoflurane-induced caspase-3 activation and a oligomerization .
	manualset3
239270	3	423467	15	NULL	NULL	NULL	NULL	oligomerization 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Anesthetic propofol attenuates the isoflurane-induced caspase-3 activation and a oligomerization .
	manualset3
239271	1	423468	15	NULL	NULL	0	NULL	Aneuploidy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Aneuploidy arising early in development is the leading genetic cause of birth defects and developmental disabilities in humans .
	manualset3
239272	2	423468	15	NULL	NULL	0	NULL	development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Aneuploidy arising early in development is the leading genetic cause of birth defects and developmental disabilities in humans .
	manualset3
239273	3	423468	15	NULL	NULL	0	NULL	genetic cause	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Aneuploidy arising early in development is the leading genetic cause of birth defects and developmental disabilities in humans .
	manualset3
239274	4	423468	15	NULL	NULL	0	NULL	birth defects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Aneuploidy arising early in development is the leading genetic cause of birth defects and developmental disabilities in humans .
	manualset3
239275	5	423468	15	NULL	NULL	0	NULL	developmental disabilities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Aneuploidy arising early in development is the leading genetic cause of birth defects and developmental disabilities in humans .
	manualset3
239276	6	423468	15	NULL	NULL	0	NULL	humans	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Aneuploidy arising early in development is the leading genetic cause of birth defects and developmental disabilities in humans .
	manualset3
239277	1	423469	15	NULL	NULL	NULL	NULL	Aneuploidy detection	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Aneuploidy detection in pigs using comparative genomic hybridization : from the oocytes to blastocysts .
	manualset3
239278	2	423469	15	NULL	NULL	0	NULL	 pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Aneuploidy detection in pigs using comparative genomic hybridization : from the oocytes to blastocysts .
	manualset3
239279	3	423469	15	NULL	NULL	0	NULL	comparative genomic hybridization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Aneuploidy detection in pigs using comparative genomic hybridization : from the oocytes to blastocysts .
	manualset3
239280	4	423469	15	NULL	NULL	NULL	NULL	oocytes 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Aneuploidy detection in pigs using comparative genomic hybridization : from the oocytes to blastocysts .
	manualset3
258248	5	423469	15	NULL	NULL	NULL	NULL	blastocysts	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Aneuploidy detection in pigs using comparative genomic hybridization : from the oocytes to blastocysts .
	manualset3
239282	1	423470	15	NULL	NULL	0	NULL	Aneurysms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Aneurysms or pseudoaneurysms of the native coronary arteries or bypass grafts are uncommon and represent a pathology with high morbidity and mortality .
	manualset3
239283	2	423470	15	NULL	NULL	0	NULL	pseudoaneurysms 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Aneurysms or pseudoaneurysms of the native coronary arteries or bypass grafts are uncommon and represent a pathology with high morbidity and mortality .
	manualset3
239284	3	423470	15	NULL	NULL	0	NULL	native coronary arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Aneurysms or pseudoaneurysms of the native coronary arteries or bypass grafts are uncommon and represent a pathology with high morbidity and mortality .
	manualset3
239285	4	423470	15	NULL	NULL	0	NULL	bypass grafts	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Aneurysms or pseudoaneurysms of the native coronary arteries or bypass grafts are uncommon and represent a pathology with high morbidity and mortality .
	manualset3
239286	5	423470	15	NULL	NULL	0	NULL	pathology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Aneurysms or pseudoaneurysms of the native coronary arteries or bypass grafts are uncommon and represent a pathology with high morbidity and mortality .
	manualset3
239287	6	423470	15	NULL	NULL	0	NULL	morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Aneurysms or pseudoaneurysms of the native coronary arteries or bypass grafts are uncommon and represent a pathology with high morbidity and mortality .
	manualset3
239288	7	423470	15	NULL	NULL	0	NULL	morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Aneurysms or pseudoaneurysms of the native coronary arteries or bypass grafts are uncommon and represent a pathology with high morbidity and mortality .
	manualset3
239289	1	423471	15	NULL	NULL	0	NULL	Dysimmune manifestations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Dysimmune manifestations in Horton 's disease and polymyalgia rheumatica ) .
	manualset3
239290	2	423471	15	NULL	NULL	0	NULL	Horton 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Dysimmune manifestations in Horton 's disease and polymyalgia rheumatica ) .
	manualset3
239291	3	423471	15	NULL	NULL	0	NULL	polymyalgia rheumatica	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Dysimmune manifestations in Horton 's disease and polymyalgia rheumatica ) .
	manualset3
239292	1	423472	15	NULL	NULL	0	NULL	Angiogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiogenesis is a promising target for cancer prevention and treatment .
	manualset3
239293	2	423472	15	NULL	NULL	0	NULL	target	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiogenesis is a promising target for cancer prevention and treatment .
	manualset3
239294	3	423472	15	NULL	NULL	0	NULL	cancer prevention 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiogenesis is a promising target for cancer prevention and treatment .
	manualset3
239295	4	423472	15	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiogenesis is a promising target for cancer prevention and treatment .
	manualset3
239296	1	423473	15	NULL	NULL	0	NULL	Angiogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiogenesis is a significant and possibly primary event in the pathogenesis of inflammatory diseases including arthritis .
	manualset3
239297	2	423473	15	NULL	NULL	0	NULL	event	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiogenesis is a significant and possibly primary event in the pathogenesis of inflammatory diseases including arthritis .
	manualset3
239298	3	423473	15	NULL	NULL	0	NULL	pathogenesis of inflammatory diseases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiogenesis is a significant and possibly primary event in the pathogenesis of inflammatory diseases including arthritis .
	manualset3
239299	4	423473	15	NULL	NULL	0	NULL	 arthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiogenesis is a significant and possibly primary event in the pathogenesis of inflammatory diseases including arthritis .
	manualset3
239300	1	423474	15	NULL	NULL	0	NULL	Angiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiography and dynamic airway evaluation with MDCT in the diagnosis of double aortic arch associated with tracheomalacia .
	manualset3
239301	2	423474	15	NULL	NULL	0	NULL	dynamic airway evaluation with MDCT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiography and dynamic airway evaluation with MDCT in the diagnosis of double aortic arch associated with tracheomalacia .
	manualset3
239302	3	423474	15	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiography and dynamic airway evaluation with MDCT in the diagnosis of double aortic arch associated with tracheomalacia .
	manualset3
239303	4	423474	15	NULL	NULL	0	NULL	double aortic arch	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiography and dynamic airway evaluation with MDCT in the diagnosis of double aortic arch associated with tracheomalacia .
	manualset3
239304	5	423474	15	NULL	NULL	0	NULL	tracheomalacia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiography and dynamic airway evaluation with MDCT in the diagnosis of double aortic arch associated with tracheomalacia .
	manualset3
239305	1	423475	15	NULL	NULL	0	NULL	Angioplasty	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Angioplasty and stenting are relatively safe and feasible tools for control of blood pressure ( BP ) in ARAS .
	manualset3
239306	2	423475	15	NULL	NULL	0	NULL	stenting	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Angioplasty and stenting are relatively safe and feasible tools for control of blood pressure ( BP ) in ARAS .
	manualset3
239307	3	423475	15	NULL	NULL	0	NULL	tools	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Angioplasty and stenting are relatively safe and feasible tools for control of blood pressure ( BP ) in ARAS .
	manualset3
239308	4	423475	15	NULL	NULL	0	NULL	control of blood pressure ( BP )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Angioplasty and stenting are relatively safe and feasible tools for control of blood pressure ( BP ) in ARAS .
	manualset3
239309	5	423475	15	NULL	NULL	0	NULL	ARAS	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Angioplasty and stenting are relatively safe and feasible tools for control of blood pressure ( BP ) in ARAS .
	manualset3
239310	1	423476	15	NULL	NULL	0	NULL	Angiotensin-converting enzyme D allele 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin-converting enzyme D allele does not influence susceptibility to acute hypoxic respiratory failure in children .
	manualset3
239311	2	423476	15	NULL	NULL	0	NULL	influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin-converting enzyme D allele does not influence susceptibility to acute hypoxic respiratory failure in children .
	manualset3
239312	3	423476	15	NULL	NULL	0	NULL	susceptibility	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin-converting enzyme D allele does not influence susceptibility to acute hypoxic respiratory failure in children .
	manualset3
239313	4	423476	15	NULL	NULL	0	NULL	acute hypoxic respiratory failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin-converting enzyme D allele does not influence susceptibility to acute hypoxic respiratory failure in children .
	manualset3
239314	5	423476	15	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin-converting enzyme D allele does not influence susceptibility to acute hypoxic respiratory failure in children .
	manualset3
239315	1	423477	15	NULL	NULL	0	NULL	Angiotensin I-converting enzyme ( ACE )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin I-converting enzyme ( ACE ) is a key enzyme in the regulation of systemic blood pressure and plays a major role in the renin-angiotensin and bradykinin-kinin systems , at the luminal surface of the vascular endothelia .
	manualset3
239316	2	423477	15	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin I-converting enzyme ( ACE ) is a key enzyme in the regulation of systemic blood pressure and plays a major role in the renin-angiotensin and bradykinin-kinin systems , at the luminal surface of the vascular endothelia .
	manualset3
239317	3	423477	15	NULL	NULL	NULL	NULL	regulation of systemic blood pressure	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Angiotensin I-converting enzyme ( ACE ) is a key enzyme in the regulation of systemic blood pressure and plays a major role in the renin-angiotensin and bradykinin-kinin systems , at the luminal surface of the vascular endothelia .
	manualset3
239318	4	423477	15	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin I-converting enzyme ( ACE ) is a key enzyme in the regulation of systemic blood pressure and plays a major role in the renin-angiotensin and bradykinin-kinin systems , at the luminal surface of the vascular endothelia .
	manualset3
239319	5	423477	15	NULL	NULL	0	NULL	renin-angiotensin system	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin I-converting enzyme ( ACE ) is a key enzyme in the regulation of systemic blood pressure and plays a major role in the renin-angiotensin and bradykinin-kinin systems , at the luminal surface of the vascular endothelia .
	manualset3
239320	6	423477	15	NULL	NULL	0	NULL	bradykinin-kinin system	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin I-converting enzyme ( ACE ) is a key enzyme in the regulation of systemic blood pressure and plays a major role in the renin-angiotensin and bradykinin-kinin systems , at the luminal surface of the vascular endothelia .
	manualset3
239321	7	423477	15	NULL	NULL	0	NULL	 luminal surface of the vascular endothelia	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin I-converting enzyme ( ACE ) is a key enzyme in the regulation of systemic blood pressure and plays a major role in the renin-angiotensin and bradykinin-kinin systems , at the luminal surface of the vascular endothelia .
	manualset3
239322	1	423478	15	NULL	NULL	0	NULL	Angiotensin II	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin II also caused a small increase in ACTH release but had no effect on the release of LH , TSH , and GH .
	manualset3
239323	2	423478	15	NULL	NULL	0	NULL	increase in ACTH release	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin II also caused a small increase in ACTH release but had no effect on the release of LH , TSH , and GH .
	manualset3
239324	3	423478	15	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin II also caused a small increase in ACTH release but had no effect on the release of LH , TSH , and GH .
	manualset3
239325	4	423478	15	NULL	NULL	0	NULL	release of LH	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin II also caused a small increase in ACTH release but had no effect on the release of LH , TSH , and GH .
	manualset3
239326	5	423478	15	NULL	NULL	0	NULL	release of TSH	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin II also caused a small increase in ACTH release but had no effect on the release of LH , TSH , and GH .
	manualset3
239327	6	423478	15	NULL	NULL	0	NULL	release of GH	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin II also caused a small increase in ACTH release but had no effect on the release of LH , TSH , and GH .
	manualset3
239328	1	423479	15	NULL	NULL	0	NULL	Dyspnea	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Dyspnea of cardial origin ) .
	manualset3
239329	2	423479	15	NULL	NULL	NULL	NULL	cardial origin	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Dyspnea of cardial origin ) .
	manualset3
239330	1	423480	15	NULL	NULL	0	NULL	Angiotensin II	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin II produced pressor and drinking responses and increased glucose utilization selectively in the subfornical organ and pituitary neural lobe and in no other brain structure .
	manualset3
239331	2	423480	15	NULL	NULL	0	NULL	pressor responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin II produced pressor and drinking responses and increased glucose utilization selectively in the subfornical organ and pituitary neural lobe and in no other brain structure .
	manualset3
239332	3	423480	15	NULL	NULL	NULL	NULL	drinking responses	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Angiotensin II produced pressor and drinking responses and increased glucose utilization selectively in the subfornical organ and pituitary neural lobe and in no other brain structure .
	manualset3
239333	4	423480	15	NULL	NULL	0	NULL	glucose utilization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin II produced pressor and drinking responses and increased glucose utilization selectively in the subfornical organ and pituitary neural lobe and in no other brain structure .
	manualset3
239334	5	423480	15	NULL	NULL	0	NULL	subfornical organ	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin II produced pressor and drinking responses and increased glucose utilization selectively in the subfornical organ and pituitary neural lobe and in no other brain structure .
	manualset3
239335	6	423480	15	NULL	NULL	0	NULL	pituitary neural lobe	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin II produced pressor and drinking responses and increased glucose utilization selectively in the subfornical organ and pituitary neural lobe and in no other brain structure .
	manualset3
239336	7	423480	15	NULL	NULL	0	NULL	brain structure	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin II produced pressor and drinking responses and increased glucose utilization selectively in the subfornical organ and pituitary neural lobe and in no other brain structure .
	manualset3
239337	1	423481	15	NULL	NULL	0	NULL	Angiotensin converting enzyme inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin converting enzyme inhibition lowers body weight and improves glucose tolerance in C57BL/6J mice maintained on a high fat diet .
	manualset3
239338	2	423481	15	NULL	NULL	0	NULL	body weight	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin converting enzyme inhibition lowers body weight and improves glucose tolerance in C57BL/6J mice maintained on a high fat diet .
	manualset3
239339	3	423481	15	NULL	NULL	0	NULL	glucose tolerance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin converting enzyme inhibition lowers body weight and improves glucose tolerance in C57BL/6J mice maintained on a high fat diet .
	manualset3
239340	4	423481	15	NULL	NULL	0	NULL	C57BL/6J mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Angiotensin converting enzyme inhibition lowers body weight and improves glucose tolerance in C57BL/6J mice maintained on a high fat diet .
	manualset3
239341	5	423481	15	NULL	NULL	NULL	NULL	high fat diet	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Angiotensin converting enzyme inhibition lowers body weight and improves glucose tolerance in C57BL/6J mice maintained on a high fat diet .
	manualset3
239342	1	423482	15	NULL	NULL	0	NULL	Angular dependences	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Angular , wavelength , and polarization dependences are investigated for the location of structural irregularities at interfaces or in the bulk of a multilayer .
	manualset3
239343	2	423482	15	NULL	NULL	0	NULL	wavelength dependences	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Angular , wavelength , and polarization dependences are investigated for the location of structural irregularities at interfaces or in the bulk of a multilayer .
	manualset3
239344	3	423482	15	NULL	NULL	0	NULL	polarization dependences 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Angular , wavelength , and polarization dependences are investigated for the location of structural irregularities at interfaces or in the bulk of a multilayer .
	manualset3
239345	4	423482	15	NULL	NULL	0	NULL	location of structural irregularities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Angular , wavelength , and polarization dependences are investigated for the location of structural irregularities at interfaces or in the bulk of a multilayer .
	manualset3
239346	5	423482	15	NULL	NULL	0	NULL	interfaces	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Angular , wavelength , and polarization dependences are investigated for the location of structural irregularities at interfaces or in the bulk of a multilayer .
	manualset3
239347	6	423482	15	NULL	NULL	NULL	NULL	bulk of a multilayer	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Angular , wavelength , and polarization dependences are investigated for the location of structural irregularities at interfaces or in the bulk of a multilayer .
	manualset3
239348	1	423483	15	NULL	NULL	0	NULL	Anhedonia	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Anhedonia and the experience of emotion in individuals with schizophrenia .
	manualset3
239349	2	423483	15	NULL	NULL	0	NULL	experience of emotion	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Anhedonia and the experience of emotion in individuals with schizophrenia .
	manualset3
239350	3	423483	15	NULL	NULL	0	NULL	individuals 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Anhedonia and the experience of emotion in individuals with schizophrenia .
	manualset3
239351	4	423483	15	NULL	NULL	0	NULL	schizophrenia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Anhedonia and the experience of emotion in individuals with schizophrenia .
	manualset3
239352	1	423484	15	NULL	NULL	0	NULL	Animal pharmacokinetic data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Animal pharmacokinetic data published elsewhere suggest that BI 397 may be dosed less frequently than teicoplanin and the results of early studies in humans are awaited with interest , especially when treating teicoplanin-refractory coagulase-negative staphylococci .
	manualset3
239353	2	423484	15	NULL	NULL	0	NULL	BI 397	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Animal pharmacokinetic data published elsewhere suggest that BI 397 may be dosed less frequently than teicoplanin and the results of early studies in humans are awaited with interest , especially when treating teicoplanin-refractory coagulase-negative staphylococci .
	manualset3
239354	3	423484	15	NULL	NULL	0	NULL	teicoplanin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Animal pharmacokinetic data published elsewhere suggest that BI 397 may be dosed less frequently than teicoplanin and the results of early studies in humans are awaited with interest , especially when treating teicoplanin-refractory coagulase-negative staphylococci .
	manualset3
239355	4	423484	15	NULL	NULL	0	NULL	results	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Animal pharmacokinetic data published elsewhere suggest that BI 397 may be dosed less frequently than teicoplanin and the results of early studies in humans are awaited with interest , especially when treating teicoplanin-refractory coagulase-negative staphylococci .
	manualset3
239356	5	423484	15	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Animal pharmacokinetic data published elsewhere suggest that BI 397 may be dosed less frequently than teicoplanin and the results of early studies in humans are awaited with interest , especially when treating teicoplanin-refractory coagulase-negative staphylococci .
	manualset3
239357	6	423484	15	NULL	NULL	0	NULL	humans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Animal pharmacokinetic data published elsewhere suggest that BI 397 may be dosed less frequently than teicoplanin and the results of early studies in humans are awaited with interest , especially when treating teicoplanin-refractory coagulase-negative staphylococci .
	manualset3
239358	7	423484	15	NULL	NULL	0	NULL	interest	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Animal pharmacokinetic data published elsewhere suggest that BI 397 may be dosed less frequently than teicoplanin and the results of early studies in humans are awaited with interest , especially when treating teicoplanin-refractory coagulase-negative staphylococci .
	manualset3
239359	8	423484	15	NULL	NULL	0	NULL	teicoplanin-refractory coagulase-negative staphylococci 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Animal pharmacokinetic data published elsewhere suggest that BI 397 may be dosed less frequently than teicoplanin and the results of early studies in humans are awaited with interest , especially when treating teicoplanin-refractory coagulase-negative staphylococci .
	manualset3
239360	1	423485	15	NULL	NULL	0	NULL	Animal models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Animal models for the study of hepatitis C virus infection and replication .
	manualset3
239361	2	423485	15	NULL	NULL	0	NULL	study of hepatitis C virus infection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Animal models for the study of hepatitis C virus infection and replication .
	manualset3
258252	3	423485	15	NULL	NULL	NULL	NULL	replication 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Animal models for the study of hepatitis C virus infection and replication .
	manualset3
239363	1	423486	15	NULL	NULL	0	NULL	Animal studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Animal studies of pre-pulse inhibition , attenuation of social interaction , and stereotypy and alterations in locomotion are used to study MAP in rodents .
	manualset3
239364	2	423486	15	NULL	NULL	NULL	NULL	pre-pulse inhibition	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Animal studies of pre-pulse inhibition , attenuation of social interaction , and stereotypy and alterations in locomotion are used to study MAP in rodents .
	manualset3
239365	3	423486	15	NULL	NULL	NULL	NULL	attenuation of social interaction	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Animal studies of pre-pulse inhibition , attenuation of social interaction , and stereotypy and alterations in locomotion are used to study MAP in rodents .
	manualset3
239366	4	423486	15	NULL	NULL	0	NULL	stereotypy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Animal studies of pre-pulse inhibition , attenuation of social interaction , and stereotypy and alterations in locomotion are used to study MAP in rodents .
	manualset3
239367	5	423486	15	NULL	NULL	0	NULL	alterations in locomotion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Animal studies of pre-pulse inhibition , attenuation of social interaction , and stereotypy and alterations in locomotion are used to study MAP in rodents .
	manualset3
239368	6	423486	15	NULL	NULL	NULL	NULL	MAP	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Animal studies of pre-pulse inhibition , attenuation of social interaction , and stereotypy and alterations in locomotion are used to study MAP in rodents .
	manualset3
239369	7	423486	15	NULL	NULL	0	NULL	rodents	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Animal studies of pre-pulse inhibition , attenuation of social interaction , and stereotypy and alterations in locomotion are used to study MAP in rodents .
	manualset3
239370	1	423487	15	NULL	NULL	0	NULL	( E ) -1 , 2 - Bis { 4 - ( dimeth-yl ( vin-yl ) silyl ) - phenyl } - ethene 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( E ) -1 , 2 - Bis { 4 - ( dimeth-yl ( vin-yl ) silyl ) - phenyl } - ethene .
	manualset3
239371	1	423488	15	NULL	NULL	0	NULL	Animal weights	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Animal weights , as well as the survival of the diabetic animals without insulin therapy , were also observed .
	manualset3
239372	2	423488	15	NULL	NULL	0	NULL	survival 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Animal weights , as well as the survival of the diabetic animals without insulin therapy , were also observed .
	manualset3
239373	3	423488	15	NULL	NULL	0	NULL	diabetic animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Animal weights , as well as the survival of the diabetic animals without insulin therapy , were also observed .
	manualset3
239374	4	423488	15	NULL	NULL	0	NULL	insulin therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Animal weights , as well as the survival of the diabetic animals without insulin therapy , were also observed .
	manualset3
239375	1	423489	15	NULL	NULL	0	NULL	Animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals in Groups 2-6 were placed on diet formulated with bread samples obtained from the five different locations in Ilorin metropolis .
	manualset3
239376	2	423489	15	NULL	NULL	0	NULL	Groups 2-6	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals in Groups 2-6 were placed on diet formulated with bread samples obtained from the five different locations in Ilorin metropolis .
	manualset3
239377	3	423489	15	NULL	NULL	0	NULL	diet 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals in Groups 2-6 were placed on diet formulated with bread samples obtained from the five different locations in Ilorin metropolis .
	manualset3
239378	4	423489	15	NULL	NULL	0	NULL	bread samples	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals in Groups 2-6 were placed on diet formulated with bread samples obtained from the five different locations in Ilorin metropolis .
	manualset3
239379	5	423489	15	NULL	NULL	0	NULL	five	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals in Groups 2-6 were placed on diet formulated with bread samples obtained from the five different locations in Ilorin metropolis .
	manualset3
239380	6	423489	15	NULL	NULL	0	NULL	locations	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals in Groups 2-6 were placed on diet formulated with bread samples obtained from the five different locations in Ilorin metropolis .
	manualset3
239381	7	423489	15	NULL	NULL	0	NULL	Ilorin metropolis 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals in Groups 2-6 were placed on diet formulated with bread samples obtained from the five different locations in Ilorin metropolis .
	manualset3
239382	1	423490	15	NULL	NULL	0	NULL	Animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals often use social information about conspecifics in making decisions about cooperation and conflict .
	manualset3
239383	2	423490	15	NULL	NULL	0	NULL	social information	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals often use social information about conspecifics in making decisions about cooperation and conflict .
	manualset3
239384	3	423490	15	NULL	NULL	0	NULL	 conspecifics	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals often use social information about conspecifics in making decisions about cooperation and conflict .
	manualset3
239385	4	423490	15	NULL	NULL	0	NULL	decisions	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals often use social information about conspecifics in making decisions about cooperation and conflict .
	manualset3
239386	5	423490	15	NULL	NULL	0	NULL	cooperation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals often use social information about conspecifics in making decisions about cooperation and conflict .
	manualset3
239387	6	423490	15	NULL	NULL	0	NULL	conflict	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals often use social information about conspecifics in making decisions about cooperation and conflict .
	manualset3
239388	1	423491	15	NULL	NULL	0	NULL	Animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals that had been subjected to cord clamping showed reduced brain volumes and dimensions on P80 .
	manualset3
239389	2	423491	15	NULL	NULL	0	NULL	cord clamping	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals that had been subjected to cord clamping showed reduced brain volumes and dimensions on P80 .
	manualset3
239390	3	423491	15	NULL	NULL	0	NULL	brain volumes	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals that had been subjected to cord clamping showed reduced brain volumes and dimensions on P80 .
	manualset3
239391	4	423491	15	NULL	NULL	0	NULL	dimensions 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals that had been subjected to cord clamping showed reduced brain volumes and dimensions on P80 .
	manualset3
239392	5	423491	15	NULL	NULL	0	NULL	P80	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals that had been subjected to cord clamping showed reduced brain volumes and dimensions on P80 .
	manualset3
239393	1	423492	15	NULL	NULL	0	NULL	Animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals treated with CEE + MPA showed significant reductions in 5-HIAA in the dorsal raphe nucleus , a significant reduction in dopamine in the hypothalamus , and a significant reduction in serotonin ( 5-HT ) levels in area 8AD of the frontal cortex .
	manualset3
239394	2	423492	15	NULL	NULL	0	NULL	CEE + MPA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals treated with CEE + MPA showed significant reductions in 5-HIAA in the dorsal raphe nucleus , a significant reduction in dopamine in the hypothalamus , and a significant reduction in serotonin ( 5-HT ) levels in area 8AD of the frontal cortex .
	manualset3
239395	3	423492	15	NULL	NULL	NULL	NULL	reductions	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Animals treated with CEE + MPA showed significant reductions in 5-HIAA in the dorsal raphe nucleus , a significant reduction in dopamine in the hypothalamus , and a significant reduction in serotonin ( 5-HT ) levels in area 8AD of the frontal cortex .
	manualset3
239396	4	423492	15	NULL	NULL	0	NULL	5-HIAA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals treated with CEE + MPA showed significant reductions in 5-HIAA in the dorsal raphe nucleus , a significant reduction in dopamine in the hypothalamus , and a significant reduction in serotonin ( 5-HT ) levels in area 8AD of the frontal cortex .
	manualset3
239397	5	423492	15	NULL	NULL	0	NULL	dorsal raphe nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals treated with CEE + MPA showed significant reductions in 5-HIAA in the dorsal raphe nucleus , a significant reduction in dopamine in the hypothalamus , and a significant reduction in serotonin ( 5-HT ) levels in area 8AD of the frontal cortex .
	manualset3
239398	6	423492	15	NULL	NULL	0	NULL	reduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals treated with CEE + MPA showed significant reductions in 5-HIAA in the dorsal raphe nucleus , a significant reduction in dopamine in the hypothalamus , and a significant reduction in serotonin ( 5-HT ) levels in area 8AD of the frontal cortex .
	manualset3
239399	7	423492	15	NULL	NULL	0	NULL	dopamine 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals treated with CEE + MPA showed significant reductions in 5-HIAA in the dorsal raphe nucleus , a significant reduction in dopamine in the hypothalamus , and a significant reduction in serotonin ( 5-HT ) levels in area 8AD of the frontal cortex .
	manualset3
239400	8	423492	15	NULL	NULL	0	NULL	hypothalamus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals treated with CEE + MPA showed significant reductions in 5-HIAA in the dorsal raphe nucleus , a significant reduction in dopamine in the hypothalamus , and a significant reduction in serotonin ( 5-HT ) levels in area 8AD of the frontal cortex .
	manualset3
239401	9	423492	15	NULL	NULL	0	NULL	reduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals treated with CEE + MPA showed significant reductions in 5-HIAA in the dorsal raphe nucleus , a significant reduction in dopamine in the hypothalamus , and a significant reduction in serotonin ( 5-HT ) levels in area 8AD of the frontal cortex .
	manualset3
239402	10	423492	15	NULL	NULL	0	NULL	serotonin ( 5-HT ) levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals treated with CEE + MPA showed significant reductions in 5-HIAA in the dorsal raphe nucleus , a significant reduction in dopamine in the hypothalamus , and a significant reduction in serotonin ( 5-HT ) levels in area 8AD of the frontal cortex .
	manualset3
239403	11	423492	15	NULL	NULL	0	NULL	area 8AD of the frontal cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals treated with CEE + MPA showed significant reductions in 5-HIAA in the dorsal raphe nucleus , a significant reduction in dopamine in the hypothalamus , and a significant reduction in serotonin ( 5-HT ) levels in area 8AD of the frontal cortex .
	manualset3
240339	1	423493	15	NULL	NULL	0	NULL	Animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240340	2	423493	15	NULL	NULL	0	NULL	treatment groups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240341	3	423493	15	NULL	NULL	0	NULL	I 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240342	4	423493	15	NULL	NULL	0	NULL	II 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240349	5	423493	15	NULL	NULL	0	NULL	Allotrap	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240351	6	423493	15	NULL	NULL	0	NULL	20 mg/kg/day	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240353	7	423493	15	NULL	NULL	0	NULL	Days 0-4	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240355	8	423493	15	NULL	NULL	0	NULL	III	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240359	9	423493	15	NULL	NULL	0	NULL	cyclosporine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240360	10	423493	15	NULL	NULL	0	NULL	CsA	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240361	11	423493	15	NULL	NULL	0	NULL	10 mg/kg/day 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240363	12	423493	15	NULL	NULL	0	NULL	Days 0-4	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240364	13	423493	15	NULL	NULL	0	NULL	IV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240365	14	423493	15	NULL	NULL	0	NULL	Allotrap 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240367	15	423493	15	NULL	NULL	0	NULL	CsA	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240370	16	423493	15	NULL	NULL	0	NULL	groups II 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240372	17	423493	15	NULL	NULL	NULL	NULL	group III	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240373	18	423493	15	NULL	NULL	0	NULL	V	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240375	19	423493	15	NULL	NULL	0	NULL	Allotrap	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240377	20	423493	15	NULL	NULL	0	NULL	40 mg/kg/day 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240380	21	423493	15	NULL	NULL	0	NULL	day	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240381	22	423493	15	NULL	NULL	0	NULL	Days -19 to 4 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240382	23	423493	15	NULL	NULL	0	NULL	VI	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240383	24	423493	15	NULL	NULL	0	NULL	Allotrap	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240384	25	423493	15	NULL	NULL	0	NULL	CsA	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240385	26	423493	15	NULL	NULL	0	NULL	groups III	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240386	27	423493	15	NULL	NULL	NULL	NULL	groups V	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240388	28	423493	15	NULL	NULL	0	NULL	VII	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240389	29	423493	15	NULL	NULL	0	NULL	Allotrap	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240390	30	423493	15	NULL	NULL	0	NULL	CsA	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240395	31	423493	15	NULL	NULL	0	NULL	groups III 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240397	32	423493	15	NULL	NULL	0	NULL	groups V	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
240399	33	423493	15	NULL	NULL	NULL	NULL	Allotrap 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
258253	34	423493	15	NULL	NULL	NULL	NULL	intragraft Days 0-4 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Animals were divided into treatment groups : I , none ; II , Allotrap ( 20 mg/kg/day on Days 0-4 ) ; III , cyclosporine ( CsA ; 10 mg/kg/day on Days 0-4 ) ; IV , Allotrap + CsA ( as in groups II and III ) ; V , Allotrap ( 40 mg/kg/day every other day on Days -19 to 4 ) ; VI , Allotrap + CsA ( as in groups III and V ) ; VII , Allotrap + CsA ( as in groups III and V , with Allotrap administered intragraft Days 0-4 ) .
	manualset3
239404	1	423494	15	NULL	NULL	0	NULL	Animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were fed a control diet or a 10 % cod liver oil ( CLO ) - enriched diet .
	manualset3
239405	2	423494	15	NULL	NULL	0	NULL	control diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were fed a control diet or a 10 % cod liver oil ( CLO ) - enriched diet .
	manualset3
239406	3	423494	15	NULL	NULL	0	NULL	10 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were fed a control diet or a 10 % cod liver oil ( CLO ) - enriched diet .
	manualset3
239407	4	423494	15	NULL	NULL	0	NULL	cod liver oil ( CLO ) - enriched diet 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were fed a control diet or a 10 % cod liver oil ( CLO ) - enriched diet .
	manualset3
239408	1	423495	15	NULL	NULL	0	NULL	Animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were killed after 14 days , and MD lesions were quantified in H & E stained slides .
	manualset3
239409	2	423495	15	NULL	NULL	0	NULL	14 days	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were killed after 14 days , and MD lesions were quantified in H & E stained slides .
	manualset3
239410	3	423495	15	NULL	NULL	0	NULL	MD lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were killed after 14 days , and MD lesions were quantified in H & E stained slides .
	manualset3
239411	4	423495	15	NULL	NULL	0	NULL	H & E stained slides	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were killed after 14 days , and MD lesions were quantified in H & E stained slides .
	manualset3
239412	1	423496	15	NULL	NULL	0	NULL	Animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were received statins orally prior to induction of inflammation by injection of carrageenan into rat paw or the pouch .
	manualset3
239413	2	423496	15	NULL	NULL	0	NULL	statins	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were received statins orally prior to induction of inflammation by injection of carrageenan into rat paw or the pouch .
	manualset3
239414	3	423496	15	NULL	NULL	0	NULL	induction of inflammation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were received statins orally prior to induction of inflammation by injection of carrageenan into rat paw or the pouch .
	manualset3
239415	4	423496	15	NULL	NULL	0	NULL	injection of carrageenan	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were received statins orally prior to induction of inflammation by injection of carrageenan into rat paw or the pouch .
	manualset3
239416	5	423496	15	NULL	NULL	0	NULL	 rat paw	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were received statins orally prior to induction of inflammation by injection of carrageenan into rat paw or the pouch .
	manualset3
239417	6	423496	15	NULL	NULL	0	NULL	pouch	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were received statins orally prior to induction of inflammation by injection of carrageenan into rat paw or the pouch .
	manualset3
239418	1	423497	15	NULL	NULL	0	NULL	Animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were sacrificed 4 and 24 hr postburn , and blood , peritoneal fluid , mesenteric lymph nodes , spleen , liver , and lungs were harvested aseptically .
	manualset3
239419	2	423497	15	NULL	NULL	0	NULL	4 hr postburn	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were sacrificed 4 and 24 hr postburn , and blood , peritoneal fluid , mesenteric lymph nodes , spleen , liver , and lungs were harvested aseptically .
	manualset3
239420	3	423497	15	NULL	NULL	0	NULL	24 hr postburn	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were sacrificed 4 and 24 hr postburn , and blood , peritoneal fluid , mesenteric lymph nodes , spleen , liver , and lungs were harvested aseptically .
	manualset3
239421	4	423497	15	NULL	NULL	0	NULL	blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were sacrificed 4 and 24 hr postburn , and blood , peritoneal fluid , mesenteric lymph nodes , spleen , liver , and lungs were harvested aseptically .
	manualset3
239422	5	423497	15	NULL	NULL	0	NULL	peritoneal fluid	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were sacrificed 4 and 24 hr postburn , and blood , peritoneal fluid , mesenteric lymph nodes , spleen , liver , and lungs were harvested aseptically .
	manualset3
239423	6	423497	15	NULL	NULL	0	NULL	mesenteric lymph nodes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were sacrificed 4 and 24 hr postburn , and blood , peritoneal fluid , mesenteric lymph nodes , spleen , liver , and lungs were harvested aseptically .
	manualset3
239424	7	423497	15	NULL	NULL	0	NULL	spleen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were sacrificed 4 and 24 hr postburn , and blood , peritoneal fluid , mesenteric lymph nodes , spleen , liver , and lungs were harvested aseptically .
	manualset3
239425	8	423497	15	NULL	NULL	0	NULL	liver 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were sacrificed 4 and 24 hr postburn , and blood , peritoneal fluid , mesenteric lymph nodes , spleen , liver , and lungs were harvested aseptically .
	manualset3
239426	9	423497	15	NULL	NULL	0	NULL	lungs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals were sacrificed 4 and 24 hr postburn , and blood , peritoneal fluid , mesenteric lymph nodes , spleen , liver , and lungs were harvested aseptically .
	manualset3
239427	1	423498	15	NULL	NULL	0	NULL	( E , Z ) - Diene 10	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( E , Z ) - Diene 10 was subjected to the nitroso Diels-Alder reaction to give the 1 , 4-trans six-membered ring adduct , 4a .
	manualset3
239428	2	423498	15	NULL	NULL	NULL	NULL	nitroso Diels-Alder reaction	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( E , Z ) - Diene 10 was subjected to the nitroso Diels-Alder reaction to give the 1 , 4-trans six-membered ring adduct , 4a .
	manualset3
239429	3	423498	15	NULL	NULL	0	NULL	1 , 4-trans six-membered ring adduct , 4a	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( E , Z ) - Diene 10 was subjected to the nitroso Diels-Alder reaction to give the 1 , 4-trans six-membered ring adduct , 4a .
	manualset3
239430	1	423499	15	NULL	NULL	0	NULL	Animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals with overt diabetes mellitus or pancreatic diseases were not included in this study .
	manualset3
239431	2	423499	15	NULL	NULL	0	NULL	diabetes mellitus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals with overt diabetes mellitus or pancreatic diseases were not included in this study .
	manualset3
239432	3	423499	15	NULL	NULL	0	NULL	pancreatic diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals with overt diabetes mellitus or pancreatic diseases were not included in this study .
	manualset3
239433	4	423499	15	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals with overt diabetes mellitus or pancreatic diseases were not included in this study .
	manualset3
239434	1	423500	15	NULL	NULL	0	NULL	Animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals with rhythmic oscillations before interventions had lower cerebral perfusion pressure and arterial pressure , lower heart rate , and higher laser Doppler signal than the others .
	manualset3
239435	2	423500	15	NULL	NULL	0	NULL	rhythmic oscillations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals with rhythmic oscillations before interventions had lower cerebral perfusion pressure and arterial pressure , lower heart rate , and higher laser Doppler signal than the others .
	manualset3
239436	3	423500	15	NULL	NULL	0	NULL	interventions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals with rhythmic oscillations before interventions had lower cerebral perfusion pressure and arterial pressure , lower heart rate , and higher laser Doppler signal than the others .
	manualset3
239437	4	423500	15	NULL	NULL	0	NULL	cerebral perfusion pressure	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals with rhythmic oscillations before interventions had lower cerebral perfusion pressure and arterial pressure , lower heart rate , and higher laser Doppler signal than the others .
	manualset3
239438	5	423500	15	NULL	NULL	0	NULL	arterial pressure 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals with rhythmic oscillations before interventions had lower cerebral perfusion pressure and arterial pressure , lower heart rate , and higher laser Doppler signal than the others .
	manualset3
239439	6	423500	15	NULL	NULL	0	NULL	heart rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals with rhythmic oscillations before interventions had lower cerebral perfusion pressure and arterial pressure , lower heart rate , and higher laser Doppler signal than the others .
	manualset3
239440	7	423500	15	NULL	NULL	0	NULL	laser Doppler signal	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals with rhythmic oscillations before interventions had lower cerebral perfusion pressure and arterial pressure , lower heart rate , and higher laser Doppler signal than the others .
	manualset3
239441	8	423500	15	NULL	NULL	0	NULL	others	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Animals with rhythmic oscillations before interventions had lower cerebral perfusion pressure and arterial pressure , lower heart rate , and higher laser Doppler signal than the others .
	manualset3
239465	1	423501	15	NULL	NULL	0	NULL	Anion replacement studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Anion replacement studies were also performed on mBest2 and mBest3 and differences were observed in their relative permeability and slope conductance to SCN - .
	manualset3
239466	2	423501	15	NULL	NULL	0	NULL	mBest2 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Anion replacement studies were also performed on mBest2 and mBest3 and differences were observed in their relative permeability and slope conductance to SCN - .
	manualset3
239467	3	423501	15	NULL	NULL	0	NULL	mBest3	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Anion replacement studies were also performed on mBest2 and mBest3 and differences were observed in their relative permeability and slope conductance to SCN - .
	manualset3
239468	4	423501	15	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Anion replacement studies were also performed on mBest2 and mBest3 and differences were observed in their relative permeability and slope conductance to SCN - .
	manualset3
239469	5	423501	15	NULL	NULL	0	NULL	relative permeability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Anion replacement studies were also performed on mBest2 and mBest3 and differences were observed in their relative permeability and slope conductance to SCN - .
	manualset3
239470	6	423501	15	NULL	NULL	0	NULL	slope conductance	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Anion replacement studies were also performed on mBest2 and mBest3 and differences were observed in their relative permeability and slope conductance to SCN - .
	manualset3
239471	7	423501	15	NULL	NULL	0	NULL	SCN -	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Anion replacement studies were also performed on mBest2 and mBest3 and differences were observed in their relative permeability and slope conductance to SCN - .
	manualset3
239472	1	423502	15	NULL	NULL	0	NULL	Annexin V	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Annexin V is an intracellular protein that lacks a hydrophobic signal peptide .
	manualset3
239473	2	423502	15	NULL	NULL	0	NULL	intracellular protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Annexin V is an intracellular protein that lacks a hydrophobic signal peptide .
	manualset3
239474	3	423502	15	NULL	NULL	0	NULL	lacks 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Annexin V is an intracellular protein that lacks a hydrophobic signal peptide .
	manualset3
239475	4	423502	15	NULL	NULL	0	NULL	hydrophobic signal peptide 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Annexin V is an intracellular protein that lacks a hydrophobic signal peptide .
	manualset3
239476	1	423503	15	NULL	NULL	0	NULL	Annexin V	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Annexin V for flow cytometric detection of phosphatidylserine expression on B cells undergoing apoptosis .
	manualset3
239477	2	423503	15	NULL	NULL	0	NULL	flow cytometric detection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Annexin V for flow cytometric detection of phosphatidylserine expression on B cells undergoing apoptosis .
	manualset3
239478	3	423503	15	NULL	NULL	0	NULL	phosphatidylserine expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Annexin V for flow cytometric detection of phosphatidylserine expression on B cells undergoing apoptosis .
	manualset3
239479	4	423503	15	NULL	NULL	0	NULL	B cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Annexin V for flow cytometric detection of phosphatidylserine expression on B cells undergoing apoptosis .
	manualset3
239480	5	423503	15	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Annexin V for flow cytometric detection of phosphatidylserine expression on B cells undergoing apoptosis .
	manualset3
239481	1	423504	15	NULL	NULL	0	NULL	odours	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Annoying odours have been stated in some areas around the airport , which were mainly attributed to the aircraft engine emissions rather than to fuel vapors .
	manualset3
239482	2	423504	15	NULL	NULL	0	NULL	areas around the airport	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Annoying odours have been stated in some areas around the airport , which were mainly attributed to the aircraft engine emissions rather than to fuel vapors .
	manualset3
239483	3	423504	15	NULL	NULL	0	NULL	aircraft engine emissions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Annoying odours have been stated in some areas around the airport , which were mainly attributed to the aircraft engine emissions rather than to fuel vapors .
	manualset3
239484	4	423504	15	NULL	NULL	0	NULL	fuel vapors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Annoying odours have been stated in some areas around the airport , which were mainly attributed to the aircraft engine emissions rather than to fuel vapors .
	manualset3
239485	1	423505	15	NULL	NULL	0	NULL	Annual changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Annual changes in serum calcium and inorganic phosphate levels and correlation with gonadal status of a freshwater murrel , Channa punctatus ( Bloch ) .
	manualset3
239486	2	423505	15	NULL	NULL	0	NULL	serum calcium levels 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Annual changes in serum calcium and inorganic phosphate levels and correlation with gonadal status of a freshwater murrel , Channa punctatus ( Bloch ) .
	manualset3
239487	3	423505	15	NULL	NULL	0	NULL	inorganic phosphate levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Annual changes in serum calcium and inorganic phosphate levels and correlation with gonadal status of a freshwater murrel , Channa punctatus ( Bloch ) .
	manualset3
239488	4	423505	15	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Annual changes in serum calcium and inorganic phosphate levels and correlation with gonadal status of a freshwater murrel , Channa punctatus ( Bloch ) .
	manualset3
239489	5	423505	15	NULL	NULL	0	NULL	gonadal status of a freshwater murrel 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Annual changes in serum calcium and inorganic phosphate levels and correlation with gonadal status of a freshwater murrel , Channa punctatus ( Bloch ) .
	manualset3
239490	6	423505	15	NULL	NULL	0	NULL	Channa punctatus ( Bloch )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Annual changes in serum calcium and inorganic phosphate levels and correlation with gonadal status of a freshwater murrel , Channa punctatus ( Bloch ) .
	manualset3
239491	1	423506	15	NULL	NULL	0	NULL	EAHFE ( Epidemiology Acute Heart Failure Emergency ) study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( EAHFE ( Epidemiology Acute Heart Failure Emergency ) study : analysis of the patients with echocardiography performed prior to an emergency visit due to an episode of acute heart failure ) .
	manualset3
239492	2	423506	15	NULL	NULL	0	NULL	analysis of the patients	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( EAHFE ( Epidemiology Acute Heart Failure Emergency ) study : analysis of the patients with echocardiography performed prior to an emergency visit due to an episode of acute heart failure ) .
	manualset3
239493	3	423506	15	NULL	NULL	0	NULL	echocardiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( EAHFE ( Epidemiology Acute Heart Failure Emergency ) study : analysis of the patients with echocardiography performed prior to an emergency visit due to an episode of acute heart failure ) .
	manualset3
239494	4	423506	15	NULL	NULL	0	NULL	emergency visit 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( EAHFE ( Epidemiology Acute Heart Failure Emergency ) study : analysis of the patients with echocardiography performed prior to an emergency visit due to an episode of acute heart failure ) .
	manualset3
239495	5	423506	15	NULL	NULL	0	NULL	episode of acute heart failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( EAHFE ( Epidemiology Acute Heart Failure Emergency ) study : analysis of the patients with echocardiography performed prior to an emergency visit due to an episode of acute heart failure ) .
	manualset3
239496	1	423507	15	NULL	NULL	0	NULL	Anomalies of the brachial plexus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Anomalies of the brachial plexus including its terminal branches as well as the course and distribution of the nerves in the upper limb have been reported in the literature .
	manualset3
239497	2	423507	15	NULL	NULL	0	NULL	terminal branches	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Anomalies of the brachial plexus including its terminal branches as well as the course and distribution of the nerves in the upper limb have been reported in the literature .
	manualset3
239498	3	423507	15	NULL	NULL	0	NULL	course of the nerves	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Anomalies of the brachial plexus including its terminal branches as well as the course and distribution of the nerves in the upper limb have been reported in the literature .
	manualset3
239499	4	423507	15	NULL	NULL	NULL	NULL	distribution of the nerves	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Anomalies of the brachial plexus including its terminal branches as well as the course and distribution of the nerves in the upper limb have been reported in the literature .
	manualset3
239500	5	423507	15	NULL	NULL	0	NULL	upper limb	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Anomalies of the brachial plexus including its terminal branches as well as the course and distribution of the nerves in the upper limb have been reported in the literature .
	manualset3
239501	6	423507	15	NULL	NULL	0	NULL	literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Anomalies of the brachial plexus including its terminal branches as well as the course and distribution of the nerves in the upper limb have been reported in the literature .
	manualset3
239502	1	423508	15	NULL	NULL	0	NULL	Anonymity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Anonymity in peer review -- time for a change ?
	manualset3
239503	2	423508	15	NULL	NULL	0	NULL	peer review	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Anonymity in peer review -- time for a change ?
	manualset3
239504	3	423508	15	NULL	NULL	0	NULL	time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Anonymity in peer review -- time for a change ?
	manualset3
239505	4	423508	15	NULL	NULL	0	NULL	change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Anonymity in peer review -- time for a change ?
	manualset3
239506	1	423509	15	NULL	NULL	0	NULL	NHL patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Another NHL patient , however , had multiple bone lesions , and died within a year .
	manualset3
239507	2	423509	15	NULL	NULL	0	NULL	multiple bone lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Another NHL patient , however , had multiple bone lesions , and died within a year .
	manualset3
239508	3	423509	15	NULL	NULL	0	NULL	year	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Another NHL patient , however , had multiple bone lesions , and died within a year .
	manualset3
239509	1	423510	15	NULL	NULL	0	NULL	investigator	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Another investigator to evaluated the clinical signs of VVS , blinded to the patients history or complaints .
	manualset3
239510	2	423510	15	NULL	NULL	0	NULL	clinical signs of VVS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Another investigator to evaluated the clinical signs of VVS , blinded to the patients history or complaints .
	manualset3
239511	3	423510	15	NULL	NULL	0	NULL	patients history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Another investigator to evaluated the clinical signs of VVS , blinded to the patients history or complaints .
	manualset3
239512	4	423510	15	NULL	NULL	0	NULL	patients complaints	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Another investigator to evaluated the clinical signs of VVS , blinded to the patients history or complaints .
	manualset3
239513	1	423511	15	NULL	NULL	0	NULL	antimicrobial peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Another novel antimicrobial peptide inhibited S. aureus 23-394 and was determined to have the sequence His-Gly-Leu-Asp-Asn-Tyr-Arg , corresponding to amino acid residues 15-21 of lysozyme .
	manualset3
239514	2	423511	15	NULL	NULL	0	NULL	S. aureus 23-394	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Another novel antimicrobial peptide inhibited S. aureus 23-394 and was determined to have the sequence His-Gly-Leu-Asp-Asn-Tyr-Arg , corresponding to amino acid residues 15-21 of lysozyme .
	manualset3
239515	3	423511	15	NULL	NULL	0	NULL	sequence His-Gly-Leu-Asp-Asn-Tyr-Arg	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Another novel antimicrobial peptide inhibited S. aureus 23-394 and was determined to have the sequence His-Gly-Leu-Asp-Asn-Tyr-Arg , corresponding to amino acid residues 15-21 of lysozyme .
	manualset3
239516	4	423511	15	NULL	NULL	0	NULL	amino acid residues 15-21 	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Another novel antimicrobial peptide inhibited S. aureus 23-394 and was determined to have the sequence His-Gly-Leu-Asp-Asn-Tyr-Arg , corresponding to amino acid residues 15-21 of lysozyme .
	manualset3
239517	5	423511	15	NULL	NULL	0	NULL	 lysozyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Another novel antimicrobial peptide inhibited S. aureus 23-394 and was determined to have the sequence His-Gly-Leu-Asp-Asn-Tyr-Arg , corresponding to amino acid residues 15-21 of lysozyme .
	manualset3
239518	1	423512	15	NULL	NULL	0	NULL	case	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( A case of miliary tuberculosis showing diffuse alveolar hemorrhage ) .
	manualset3
239519	2	423512	15	NULL	NULL	0	NULL	miliary tuberculosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( A case of miliary tuberculosis showing diffuse alveolar hemorrhage ) .
	manualset3
239520	3	423512	15	NULL	NULL	0	NULL	diffuse alveolar hemorrhage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( A case of miliary tuberculosis showing diffuse alveolar hemorrhage ) .
	manualset3
239521	1	423513	15	NULL	NULL	0	NULL	application 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Another possible application is the detection of dimers formed by partially self-complementary sequences .
	manualset3
239522	2	423513	15	NULL	NULL	0	NULL	detection of dimers	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Another possible application is the detection of dimers formed by partially self-complementary sequences .
	manualset3
239523	3	423513	15	NULL	NULL	NULL	NULL	self-complementary sequences	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Another possible application is the detection of dimers formed by partially self-complementary sequences .
	manualset3
239524	1	423514	15	NULL	NULL	0	NULL	mechanism 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Another possible mechanism comprehends spreading of inflammatory process through bone fissures , congenital bone malformations of due to thrombophlebitis .
	manualset3
239525	2	423514	15	NULL	NULL	0	NULL	spreading of inflammatory process	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Another possible mechanism comprehends spreading of inflammatory process through bone fissures , congenital bone malformations of due to thrombophlebitis .
	manualset3
239526	3	423514	15	NULL	NULL	0	NULL	bone fissures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Another possible mechanism comprehends spreading of inflammatory process through bone fissures , congenital bone malformations of due to thrombophlebitis .
	manualset3
239527	4	423514	15	NULL	NULL	0	NULL	congenital bone malformations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Another possible mechanism comprehends spreading of inflammatory process through bone fissures , congenital bone malformations of due to thrombophlebitis .
	manualset3
239528	5	423514	15	NULL	NULL	0	NULL	thrombophlebitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Another possible mechanism comprehends spreading of inflammatory process through bone fissures , congenital bone malformations of due to thrombophlebitis .
	manualset3
239529	1	423515	15	NULL	NULL	0	NULL	progestin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Another progestin-only injectable , NET EN ( norethindrone enanthate ) , is taken every 2 months .
	manualset3
239530	2	423515	15	NULL	NULL	0	NULL	NET EN ( norethindrone enanthate )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Another progestin-only injectable , NET EN ( norethindrone enanthate ) , is taken every 2 months .
	manualset3
239531	3	423515	15	NULL	NULL	0	NULL	2 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Another progestin-only injectable , NET EN ( norethindrone enanthate ) , is taken every 2 months .
	manualset3
239532	1	423516	15	NULL	NULL	0	NULL	phosphorylation sites	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Another set of phosphorylation sites on MAP1B are named mode II sites , and their phosphorylation is possibly due to casein kinase II .
	manualset3
239533	2	423516	15	NULL	NULL	0	NULL	MAP1B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Another set of phosphorylation sites on MAP1B are named mode II sites , and their phosphorylation is possibly due to casein kinase II .
	manualset3
239535	3	423516	15	NULL	NULL	0	NULL	mode II sites	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Another set of phosphorylation sites on MAP1B are named mode II sites , and their phosphorylation is possibly due to casein kinase II .
	manualset3
239536	4	423516	15	NULL	NULL	0	NULL	phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Another set of phosphorylation sites on MAP1B are named mode II sites , and their phosphorylation is possibly due to casein kinase II .
	manualset3
239537	5	423516	15	NULL	NULL	0	NULL	casein kinase II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Another set of phosphorylation sites on MAP1B are named mode II sites , and their phosphorylation is possibly due to casein kinase II .
	manualset3
239538	1	423517	15	NULL	NULL	0	NULL	source of risk	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Another source of risk in closed-loop systems is suboptimal performance of amperometric glucose sensors .
	manualset3
239539	2	423517	15	NULL	NULL	0	NULL	closed-loop systems	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Another source of risk in closed-loop systems is suboptimal performance of amperometric glucose sensors .
	manualset3
239540	3	423517	15	NULL	NULL	0	NULL	suboptimal performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Another source of risk in closed-loop systems is suboptimal performance of amperometric glucose sensors .
	manualset3
239541	4	423517	15	NULL	NULL	0	NULL	amperometric glucose sensors	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Another source of risk in closed-loop systems is suboptimal performance of amperometric glucose sensors .
	manualset3
239542	1	423518	15	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Another study conducted in the southern region also indicated that 13.8 % of pregnant women were anaemic caused by iron deficiency ( Phatthanapreechakul et al. 1997 ) .
	manualset3
239543	2	423518	15	NULL	NULL	0	NULL	southern region	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Another study conducted in the southern region also indicated that 13.8 % of pregnant women were anaemic caused by iron deficiency ( Phatthanapreechakul et al. 1997 ) .
	manualset3
239544	3	423518	15	NULL	NULL	0	NULL	13.8 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Another study conducted in the southern region also indicated that 13.8 % of pregnant women were anaemic caused by iron deficiency ( Phatthanapreechakul et al. 1997 ) .
	manualset3
239545	4	423518	15	NULL	NULL	0	NULL	pregnant women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Another study conducted in the southern region also indicated that 13.8 % of pregnant women were anaemic caused by iron deficiency ( Phatthanapreechakul et al. 1997 ) .
	manualset3
239546	5	423518	15	NULL	NULL	0	NULL	anaemic 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Another study conducted in the southern region also indicated that 13.8 % of pregnant women were anaemic caused by iron deficiency ( Phatthanapreechakul et al. 1997 ) .
	manualset3
239547	6	423518	15	NULL	NULL	0	NULL	iron deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Another study conducted in the southern region also indicated that 13.8 % of pregnant women were anaemic caused by iron deficiency ( Phatthanapreechakul et al. 1997 ) .
	manualset3
239548	7	423518	15	NULL	NULL	0	NULL	Phatthanapreechakul et al.	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Another study conducted in the southern region also indicated that 13.8 % of pregnant women were anaemic caused by iron deficiency ( Phatthanapreechakul et al. 1997 ) .
	manualset3
239549	8	423518	15	NULL	NULL	0	NULL	1997	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Another study conducted in the southern region also indicated that 13.8 % of pregnant women were anaemic caused by iron deficiency ( Phatthanapreechakul et al. 1997 ) .
	manualset3
239550	1	423519	15	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Another two SNPs ( rs7968902 and rs7968682 ) , which were in high linkage disequilibrium with rs1042725 , also achieved the significance level in both Caucasian populations ( overall P = 6.34 x 10 ( -7 ) , and 2.72 x 10 ( -9 ) , respectively ) .
	manualset3
239551	2	423519	15	NULL	NULL	NULL	NULL	SNPs ( rs7968902 and rs7968682 )	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Another two SNPs ( rs7968902 and rs7968682 ) , which were in high linkage disequilibrium with rs1042725 , also achieved the significance level in both Caucasian populations ( overall P = 6.34 x 10 ( -7 ) , and 2.72 x 10 ( -9 ) , respectively ) .
	manualset3
239552	3	423519	15	NULL	NULL	NULL	NULL	linkage disequilibrium	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Another two SNPs ( rs7968902 and rs7968682 ) , which were in high linkage disequilibrium with rs1042725 , also achieved the significance level in both Caucasian populations ( overall P = 6.34 x 10 ( -7 ) , and 2.72 x 10 ( -9 ) , respectively ) .
	manualset3
239553	4	423519	15	NULL	NULL	NULL	NULL	 rs1042725	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Another two SNPs ( rs7968902 and rs7968682 ) , which were in high linkage disequilibrium with rs1042725 , also achieved the significance level in both Caucasian populations ( overall P = 6.34 x 10 ( -7 ) , and 2.72 x 10 ( -9 ) , respectively ) .
	manualset3
239554	5	423519	15	NULL	NULL	0	NULL	significance level	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Another two SNPs ( rs7968902 and rs7968682 ) , which were in high linkage disequilibrium with rs1042725 , also achieved the significance level in both Caucasian populations ( overall P = 6.34 x 10 ( -7 ) , and 2.72 x 10 ( -9 ) , respectively ) .
	manualset3
239555	6	423519	15	NULL	NULL	0	NULL	Caucasian populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Another two SNPs ( rs7968902 and rs7968682 ) , which were in high linkage disequilibrium with rs1042725 , also achieved the significance level in both Caucasian populations ( overall P = 6.34 x 10 ( -7 ) , and 2.72 x 10 ( -9 ) , respectively ) .
	manualset3
239556	7	423519	15	NULL	NULL	0	NULL	P = 6.34 x 10 ( -7 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Another two SNPs ( rs7968902 and rs7968682 ) , which were in high linkage disequilibrium with rs1042725 , also achieved the significance level in both Caucasian populations ( overall P = 6.34 x 10 ( -7 ) , and 2.72 x 10 ( -9 ) , respectively ) .
	manualset3
239557	8	423519	15	NULL	NULL	0	NULL	P = 2.72 x 10 ( -9 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Another two SNPs ( rs7968902 and rs7968682 ) , which were in high linkage disequilibrium with rs1042725 , also achieved the significance level in both Caucasian populations ( overall P = 6.34 x 10 ( -7 ) , and 2.72 x 10 ( -9 ) , respectively ) .
	manualset3
239558	1	423520	15	NULL	NULL	NULL	NULL	EFFECT OF ROENTGEN IRRADIATION	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( EFFECT OF ROENTGEN IRRADIATION ON THE MOLECULAR STRUCTURE OF DNA IN SOLUTIONS ) .
	manualset3
239559	2	423520	15	NULL	NULL	0	NULL	MOLECULAR STRUCTURE OF DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	( EFFECT OF ROENTGEN IRRADIATION ON THE MOLECULAR STRUCTURE OF DNA IN SOLUTIONS ) .
	manualset3
239560	3	423520	15	NULL	NULL	0	NULL	SOLUTIONS	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	( EFFECT OF ROENTGEN IRRADIATION ON THE MOLECULAR STRUCTURE OF DNA IN SOLUTIONS ) .
	manualset3
239561	1	423521	15	NULL	NULL	0	NULL	way	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Another way to apply the serum bactericidal test is to compare the activity of different antibiotics in volunteers .
	manualset3
239562	2	423521	15	NULL	NULL	NULL	NULL	serum bactericidal test	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Another way to apply the serum bactericidal test is to compare the activity of different antibiotics in volunteers .
	manualset3
239563	3	423521	15	NULL	NULL	0	NULL	activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Another way to apply the serum bactericidal test is to compare the activity of different antibiotics in volunteers .
	manualset3
239564	4	423521	15	NULL	NULL	0	NULL	antibiotics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Another way to apply the serum bactericidal test is to compare the activity of different antibiotics in volunteers .
	manualset3
239565	5	423521	15	NULL	NULL	0	NULL	volunteers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Another way to apply the serum bactericidal test is to compare the activity of different antibiotics in volunteers .
	manualset3
239566	1	423522	15	NULL	NULL	0	NULL	Anoxia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Anoxia modulates the expression of molecules associated with endothelial dysfunction and vascular diseases .
	manualset3
239567	2	423522	15	NULL	NULL	NULL	NULL	expression of molecules	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Anoxia modulates the expression of molecules associated with endothelial dysfunction and vascular diseases .
	manualset3
239568	3	423522	15	NULL	NULL	0	NULL	endothelial dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Anoxia modulates the expression of molecules associated with endothelial dysfunction and vascular diseases .
	manualset3
239569	4	423522	15	NULL	NULL	0	NULL	vascular diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Anoxia modulates the expression of molecules associated with endothelial dysfunction and vascular diseases .
	manualset3
239570	1	423523	15	NULL	NULL	0	NULL	Anoxia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Anoxia failed to induce HsfA2 target proteins in wild-type seedlings , while overexpression of HsfA2 resulted in the production of HsfA2 targets under anoxia , correlating well with the low anoxia tolerance experiments .
	manualset3
239571	2	423523	15	NULL	NULL	0	NULL	HsfA2 target proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Anoxia failed to induce HsfA2 target proteins in wild-type seedlings , while overexpression of HsfA2 resulted in the production of HsfA2 targets under anoxia , correlating well with the low anoxia tolerance experiments .
	manualset3
239572	3	423523	15	NULL	NULL	0	NULL	wild-type seedlings	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Anoxia failed to induce HsfA2 target proteins in wild-type seedlings , while overexpression of HsfA2 resulted in the production of HsfA2 targets under anoxia , correlating well with the low anoxia tolerance experiments .
	manualset3
239573	4	423523	15	NULL	NULL	0	NULL	overexpression of HsfA2	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Anoxia failed to induce HsfA2 target proteins in wild-type seedlings , while overexpression of HsfA2 resulted in the production of HsfA2 targets under anoxia , correlating well with the low anoxia tolerance experiments .
	manualset3
239574	5	423523	15	NULL	NULL	0	NULL	production of HsfA2 targets	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Anoxia failed to induce HsfA2 target proteins in wild-type seedlings , while overexpression of HsfA2 resulted in the production of HsfA2 targets under anoxia , correlating well with the low anoxia tolerance experiments .
	manualset3
239575	6	423523	15	NULL	NULL	0	NULL	anoxia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Anoxia failed to induce HsfA2 target proteins in wild-type seedlings , while overexpression of HsfA2 resulted in the production of HsfA2 targets under anoxia , correlating well with the low anoxia tolerance experiments .
	manualset3
239576	7	423523	15	NULL	NULL	0	NULL	anoxia tolerance experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Anoxia failed to induce HsfA2 target proteins in wild-type seedlings , while overexpression of HsfA2 resulted in the production of HsfA2 targets under anoxia , correlating well with the low anoxia tolerance experiments .
	manualset3
239577	1	423524	15	NULL	NULL	0	NULL	Antagonistic effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antagonistic effects of pentagastrin and cortisol on plasma level , urinary excretion and hepatic and renal uptake of vitamin B12 after intravenous injection in the cat ( proceedings ) .
	manualset3
239578	2	423524	15	NULL	NULL	0	NULL	pentagastrin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Antagonistic effects of pentagastrin and cortisol on plasma level , urinary excretion and hepatic and renal uptake of vitamin B12 after intravenous injection in the cat ( proceedings ) .
	manualset3
239579	3	423524	15	NULL	NULL	NULL	NULL	cortisol 	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Antagonistic effects of pentagastrin and cortisol on plasma level , urinary excretion and hepatic and renal uptake of vitamin B12 after intravenous injection in the cat ( proceedings ) .
	manualset3
239580	4	423524	15	NULL	NULL	0	NULL	plasma level	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Antagonistic effects of pentagastrin and cortisol on plasma level , urinary excretion and hepatic and renal uptake of vitamin B12 after intravenous injection in the cat ( proceedings ) .
	manualset3
239581	5	423524	15	NULL	NULL	0	NULL	urinary excretion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antagonistic effects of pentagastrin and cortisol on plasma level , urinary excretion and hepatic and renal uptake of vitamin B12 after intravenous injection in the cat ( proceedings ) .
	manualset3
239582	6	423524	15	NULL	NULL	0	NULL	hepatic uptake of vitamin B12	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antagonistic effects of pentagastrin and cortisol on plasma level , urinary excretion and hepatic and renal uptake of vitamin B12 after intravenous injection in the cat ( proceedings ) .
	manualset3
239583	7	423524	15	NULL	NULL	0	NULL	renal uptake of vitamin B12	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antagonistic effects of pentagastrin and cortisol on plasma level , urinary excretion and hepatic and renal uptake of vitamin B12 after intravenous injection in the cat ( proceedings ) .
	manualset3
239584	8	423524	15	NULL	NULL	0	NULL	intravenous injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Antagonistic effects of pentagastrin and cortisol on plasma level , urinary excretion and hepatic and renal uptake of vitamin B12 after intravenous injection in the cat ( proceedings ) .
	manualset3
239585	9	423524	15	NULL	NULL	0	NULL	 cat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Antagonistic effects of pentagastrin and cortisol on plasma level , urinary excretion and hepatic and renal uptake of vitamin B12 after intravenous injection in the cat ( proceedings ) .
	manualset3
239586	10	423524	15	NULL	NULL	0	NULL	 proceedings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Antagonistic effects of pentagastrin and cortisol on plasma level , urinary excretion and hepatic and renal uptake of vitamin B12 after intravenous injection in the cat ( proceedings ) .
	manualset3
239587	1	423525	15	NULL	NULL	0	NULL	Antenatal minimal hydronephrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antenatal minimal hydronephrosis : is its follow-up an unnecessary cause of concern ?
	manualset3
239588	2	423525	15	NULL	NULL	0	NULL	follow-up	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Antenatal minimal hydronephrosis : is its follow-up an unnecessary cause of concern ?
	manualset3
239589	3	423525	15	NULL	NULL	0	NULL	cause of concern	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antenatal minimal hydronephrosis : is its follow-up an unnecessary cause of concern ?
	manualset3
239610	1	423526	15	NULL	NULL	0	NULL	Anterior axial ultrasound	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Anterior axial ultrasound in monitoring infants with Pavlik harness .
	manualset3
239611	2	423526	15	NULL	NULL	0	NULL	monitoring infants	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Anterior axial ultrasound in monitoring infants with Pavlik harness .
	manualset3
239612	3	423526	15	NULL	NULL	0	NULL	Pavlik harness	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Anterior axial ultrasound in monitoring infants with Pavlik harness .
	manualset3
239613	1	423527	15	NULL	NULL	0	NULL	Anterior stabilization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Anterior stabilization of pathologic dens fractures .
	manualset3
239614	2	423527	15	NULL	NULL	0	NULL	pathologic dens fractures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Anterior stabilization of pathologic dens fractures .
	manualset3
239615	1	423528	15	NULL	NULL	0	NULL	Anthranilate synthase ( chorismate pyruvatelyase ( amino-accepting ) , E.C. 4.1.3.27 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Anthranilate synthase ( chorismate pyruvatelyase ( amino-accepting ) , E.C. 4.1.3.27 ) catalyzes the formation of anthranilate ( o-aminobenzoate ) and pyruvic acid from chorismate and glutamine .
	manualset3
239616	2	423528	15	NULL	NULL	0	NULL	formation of anthranilate ( o-aminobenzoate ) 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Anthranilate synthase ( chorismate pyruvatelyase ( amino-accepting ) , E.C. 4.1.3.27 ) catalyzes the formation of anthranilate ( o-aminobenzoate ) and pyruvic acid from chorismate and glutamine .
	manualset3
239617	3	423528	15	NULL	NULL	NULL	NULL	formation of pyruvic acid	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Anthranilate synthase ( chorismate pyruvatelyase ( amino-accepting ) , E.C. 4.1.3.27 ) catalyzes the formation of anthranilate ( o-aminobenzoate ) and pyruvic acid from chorismate and glutamine .
	manualset3
239619	4	423528	15	NULL	NULL	NULL	NULL	 chorismate	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Anthranilate synthase ( chorismate pyruvatelyase ( amino-accepting ) , E.C. 4.1.3.27 ) catalyzes the formation of anthranilate ( o-aminobenzoate ) and pyruvic acid from chorismate and glutamine .
	manualset3
239620	5	423528	15	NULL	NULL	NULL	NULL	glutamine	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Anthranilate synthase ( chorismate pyruvatelyase ( amino-accepting ) , E.C. 4.1.3.27 ) catalyzes the formation of anthranilate ( o-aminobenzoate ) and pyruvic acid from chorismate and glutamine .
	manualset3
239621	1	423529	15	NULL	NULL	0	NULL	Anti-SRBC antibody responses 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-SRBC antibody responses stimulated by intraperitoneal or intravenous immunization with SRBC failed to augment when TGF-beta-depleted human milk was given orally .
	manualset3
239622	2	423529	15	NULL	NULL	0	NULL	intraperitoneal immunization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-SRBC antibody responses stimulated by intraperitoneal or intravenous immunization with SRBC failed to augment when TGF-beta-depleted human milk was given orally .
	manualset3
239623	3	423529	15	NULL	NULL	0	NULL	intravenous immunization 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-SRBC antibody responses stimulated by intraperitoneal or intravenous immunization with SRBC failed to augment when TGF-beta-depleted human milk was given orally .
	manualset3
239624	4	423529	15	NULL	NULL	0	NULL	SRBC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-SRBC antibody responses stimulated by intraperitoneal or intravenous immunization with SRBC failed to augment when TGF-beta-depleted human milk was given orally .
	manualset3
239625	5	423529	15	NULL	NULL	0	NULL	augment	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-SRBC antibody responses stimulated by intraperitoneal or intravenous immunization with SRBC failed to augment when TGF-beta-depleted human milk was given orally .
	manualset3
239626	6	423529	15	NULL	NULL	0	NULL	TGF-beta-depleted human milk	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-SRBC antibody responses stimulated by intraperitoneal or intravenous immunization with SRBC failed to augment when TGF-beta-depleted human milk was given orally .
	manualset3
239627	1	423530	15	NULL	NULL	0	NULL	Anti-abortion groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-abortion groups successfully blocked the availability of RU-486 in the US until President Clinton instructed his administration to promote the testing , licensing , and manufacture of the drug .
	manualset3
239628	2	423530	15	NULL	NULL	0	NULL	availability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-abortion groups successfully blocked the availability of RU-486 in the US until President Clinton instructed his administration to promote the testing , licensing , and manufacture of the drug .
	manualset3
239629	3	423530	15	NULL	NULL	NULL	NULL	RU-486	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Anti-abortion groups successfully blocked the availability of RU-486 in the US until President Clinton instructed his administration to promote the testing , licensing , and manufacture of the drug .
	manualset3
239630	4	423530	15	NULL	NULL	0	NULL	US	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-abortion groups successfully blocked the availability of RU-486 in the US until President Clinton instructed his administration to promote the testing , licensing , and manufacture of the drug .
	manualset3
239631	5	423530	15	NULL	NULL	0	NULL	President Clinton	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-abortion groups successfully blocked the availability of RU-486 in the US until President Clinton instructed his administration to promote the testing , licensing , and manufacture of the drug .
	manualset3
239632	6	423530	15	NULL	NULL	0	NULL	administration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-abortion groups successfully blocked the availability of RU-486 in the US until President Clinton instructed his administration to promote the testing , licensing , and manufacture of the drug .
	manualset3
239633	7	423530	15	NULL	NULL	0	NULL	testing of the drug	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-abortion groups successfully blocked the availability of RU-486 in the US until President Clinton instructed his administration to promote the testing , licensing , and manufacture of the drug .
	manualset3
239634	8	423530	15	NULL	NULL	0	NULL	licensing of the drug	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-abortion groups successfully blocked the availability of RU-486 in the US until President Clinton instructed his administration to promote the testing , licensing , and manufacture of the drug .
	manualset3
239635	9	423530	15	NULL	NULL	0	NULL	manufacture of the drug	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-abortion groups successfully blocked the availability of RU-486 in the US until President Clinton instructed his administration to promote the testing , licensing , and manufacture of the drug .
	manualset3
239636	1	423531	15	NULL	NULL	0	NULL	Anti-p200 pemphigoid	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-p200 pemphigoid is an autoimmune subepidermal blistering disease characterized by autoantibodies to an unknown 200-kDa acidic noncollagenous glycoprotein of the lower lamina lucida , whereas antilaminin 5 mucous membrane pemphigoid is characterized by autoantibodies to a major basement membrane extracellular matrix , laminin 5 .
	manualset3
239637	2	423531	15	NULL	NULL	0	NULL	autoimmune subepidermal blistering disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-p200 pemphigoid is an autoimmune subepidermal blistering disease characterized by autoantibodies to an unknown 200-kDa acidic noncollagenous glycoprotein of the lower lamina lucida , whereas antilaminin 5 mucous membrane pemphigoid is characterized by autoantibodies to a major basement membrane extracellular matrix , laminin 5 .
	manualset3
239638	3	423531	15	NULL	NULL	0	NULL	autoantibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-p200 pemphigoid is an autoimmune subepidermal blistering disease characterized by autoantibodies to an unknown 200-kDa acidic noncollagenous glycoprotein of the lower lamina lucida , whereas antilaminin 5 mucous membrane pemphigoid is characterized by autoantibodies to a major basement membrane extracellular matrix , laminin 5 .
	manualset3
239639	4	423531	15	NULL	NULL	NULL	NULL	200-kDa 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Anti-p200 pemphigoid is an autoimmune subepidermal blistering disease characterized by autoantibodies to an unknown 200-kDa acidic noncollagenous glycoprotein of the lower lamina lucida , whereas antilaminin 5 mucous membrane pemphigoid is characterized by autoantibodies to a major basement membrane extracellular matrix , laminin 5 .
	manualset3
239640	5	423531	15	NULL	NULL	0	NULL	acidic noncollagenous glycoprotein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-p200 pemphigoid is an autoimmune subepidermal blistering disease characterized by autoantibodies to an unknown 200-kDa acidic noncollagenous glycoprotein of the lower lamina lucida , whereas antilaminin 5 mucous membrane pemphigoid is characterized by autoantibodies to a major basement membrane extracellular matrix , laminin 5 .
	manualset3
239641	6	423531	15	NULL	NULL	0	NULL	lower lamina lucida	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-p200 pemphigoid is an autoimmune subepidermal blistering disease characterized by autoantibodies to an unknown 200-kDa acidic noncollagenous glycoprotein of the lower lamina lucida , whereas antilaminin 5 mucous membrane pemphigoid is characterized by autoantibodies to a major basement membrane extracellular matrix , laminin 5 .
	manualset3
239642	7	423531	15	NULL	NULL	0	NULL	antilaminin 5 mucous membrane pemphigoid	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-p200 pemphigoid is an autoimmune subepidermal blistering disease characterized by autoantibodies to an unknown 200-kDa acidic noncollagenous glycoprotein of the lower lamina lucida , whereas antilaminin 5 mucous membrane pemphigoid is characterized by autoantibodies to a major basement membrane extracellular matrix , laminin 5 .
	manualset3
239643	8	423531	15	NULL	NULL	0	NULL	autoantibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-p200 pemphigoid is an autoimmune subepidermal blistering disease characterized by autoantibodies to an unknown 200-kDa acidic noncollagenous glycoprotein of the lower lamina lucida , whereas antilaminin 5 mucous membrane pemphigoid is characterized by autoantibodies to a major basement membrane extracellular matrix , laminin 5 .
	manualset3
239644	9	423531	15	NULL	NULL	0	NULL	major basement membrane extracellular matrix	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-p200 pemphigoid is an autoimmune subepidermal blistering disease characterized by autoantibodies to an unknown 200-kDa acidic noncollagenous glycoprotein of the lower lamina lucida , whereas antilaminin 5 mucous membrane pemphigoid is characterized by autoantibodies to a major basement membrane extracellular matrix , laminin 5 .
	manualset3
239645	10	423531	15	NULL	NULL	0	NULL	laminin 5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-p200 pemphigoid is an autoimmune subepidermal blistering disease characterized by autoantibodies to an unknown 200-kDa acidic noncollagenous glycoprotein of the lower lamina lucida , whereas antilaminin 5 mucous membrane pemphigoid is characterized by autoantibodies to a major basement membrane extracellular matrix , laminin 5 .
	manualset3
239646	1	423532	15	NULL	NULL	0	NULL	Anti-spike agents	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-spike agents may also be of benefit in ameliorating the cognitive dysfunctions associated with epilepsy , to which spike activity may contribute .
	manualset3
239647	3	423532	15	NULL	NULL	NULL	NULL	cognitive dysfunctions 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Anti-spike agents may also be of benefit in ameliorating the cognitive dysfunctions associated with epilepsy , to which spike activity may contribute .
	manualset3
239648	4	423532	15	NULL	NULL	NULL	NULL	epilepsy	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Anti-spike agents may also be of benefit in ameliorating the cognitive dysfunctions associated with epilepsy , to which spike activity may contribute .
	manualset3
239649	5	423532	15	NULL	NULL	NULL	NULL	spike activity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Anti-spike agents may also be of benefit in ameliorating the cognitive dysfunctions associated with epilepsy , to which spike activity may contribute .
	manualset3
239650	2	423532	15	NULL	NULL	0	NULL	benefit	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Anti-spike agents may also be of benefit in ameliorating the cognitive dysfunctions associated with epilepsy , to which spike activity may contribute .
	manualset3
239651	1	423533	15	NULL	NULL	0	NULL	Antibiotic-resistant coliforms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic-resistant coliforms have been isolated from carcases , fresh and cooked meat , raw meat handlers and livestock handlers .
	manualset3
239652	2	423533	15	NULL	NULL	0	NULL	carcases	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic-resistant coliforms have been isolated from carcases , fresh and cooked meat , raw meat handlers and livestock handlers .
	manualset3
239653	3	423533	15	NULL	NULL	0	NULL	fresh meat 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic-resistant coliforms have been isolated from carcases , fresh and cooked meat , raw meat handlers and livestock handlers .
	manualset3
239654	4	423533	15	NULL	NULL	0	NULL	cooked meat	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic-resistant coliforms have been isolated from carcases , fresh and cooked meat , raw meat handlers and livestock handlers .
	manualset3
239655	5	423533	15	NULL	NULL	0	NULL	raw meat handlers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic-resistant coliforms have been isolated from carcases , fresh and cooked meat , raw meat handlers and livestock handlers .
	manualset3
239656	6	423533	15	NULL	NULL	0	NULL	livestock handlers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic-resistant coliforms have been isolated from carcases , fresh and cooked meat , raw meat handlers and livestock handlers .
	manualset3
239666	1	423534	15	NULL	NULL	0	NULL	Antibiotic-treated termites 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic-treated termites and control ( N ( 2 ) - fixing ) termites were exposed to different concentrations of dietary N ( 0 , 0.21 , and 0.94 % N ) , their ( 15 ) N signatures were obtained , and the percent nitrogen derived from the atmosphere within termite samples was calculated .
	manualset3
239667	2	423534	15	NULL	NULL	0	NULL	control ( N ( 2 ) - fixing ) termites	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic-treated termites and control ( N ( 2 ) - fixing ) termites were exposed to different concentrations of dietary N ( 0 , 0.21 , and 0.94 % N ) , their ( 15 ) N signatures were obtained , and the percent nitrogen derived from the atmosphere within termite samples was calculated .
	manualset3
239668	3	423534	15	NULL	NULL	NULL	NULL	concentrations 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Antibiotic-treated termites and control ( N ( 2 ) - fixing ) termites were exposed to different concentrations of dietary N ( 0 , 0.21 , and 0.94 % N ) , their ( 15 ) N signatures were obtained , and the percent nitrogen derived from the atmosphere within termite samples was calculated .
	manualset3
239669	4	423534	15	NULL	NULL	0	NULL	 dietary N ( 0 , 0.21 , and 0.94 % N )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic-treated termites and control ( N ( 2 ) - fixing ) termites were exposed to different concentrations of dietary N ( 0 , 0.21 , and 0.94 % N ) , their ( 15 ) N signatures were obtained , and the percent nitrogen derived from the atmosphere within termite samples was calculated .
	manualset3
239670	5	423534	15	NULL	NULL	0	NULL	( 15 ) N signatures	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic-treated termites and control ( N ( 2 ) - fixing ) termites were exposed to different concentrations of dietary N ( 0 , 0.21 , and 0.94 % N ) , their ( 15 ) N signatures were obtained , and the percent nitrogen derived from the atmosphere within termite samples was calculated .
	manualset3
239671	6	423534	15	NULL	NULL	0	NULL	percent nitrogen	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic-treated termites and control ( N ( 2 ) - fixing ) termites were exposed to different concentrations of dietary N ( 0 , 0.21 , and 0.94 % N ) , their ( 15 ) N signatures were obtained , and the percent nitrogen derived from the atmosphere within termite samples was calculated .
	manualset3
239672	7	423534	15	NULL	NULL	0	NULL	atmosphere 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic-treated termites and control ( N ( 2 ) - fixing ) termites were exposed to different concentrations of dietary N ( 0 , 0.21 , and 0.94 % N ) , their ( 15 ) N signatures were obtained , and the percent nitrogen derived from the atmosphere within termite samples was calculated .
	manualset3
239673	8	423534	15	NULL	NULL	0	NULL	termite samples	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic-treated termites and control ( N ( 2 ) - fixing ) termites were exposed to different concentrations of dietary N ( 0 , 0.21 , and 0.94 % N ) , their ( 15 ) N signatures were obtained , and the percent nitrogen derived from the atmosphere within termite samples was calculated .
	manualset3
239746	1	423535	15	NULL	NULL	0	NULL	ERP ( early recepter potentials ) 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( ERP ( early recepter potentials ) of the human eye .
	manualset3
239747	2	423535	15	NULL	NULL	0	NULL	human eye	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( ERP ( early recepter potentials ) of the human eye .
	manualset3
239748	1	423536	15	NULL	NULL	0	NULL	Antibiotic residues	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic residues in surface soils can lead to serious health risks and ecological hazards .
	manualset3
239749	2	423536	15	NULL	NULL	0	NULL	surface soils	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic residues in surface soils can lead to serious health risks and ecological hazards .
	manualset3
239750	3	423536	15	NULL	NULL	0	NULL	serious health risks 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic residues in surface soils can lead to serious health risks and ecological hazards .
	manualset3
239751	4	423536	15	NULL	NULL	0	NULL	ecological hazards	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic residues in surface soils can lead to serious health risks and ecological hazards .
	manualset3
239752	1	423537	15	NULL	NULL	0	NULL	Antibiotic resistance mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic resistance mechanisms reported in Gram-negative bacteria are causing a worldwide health problem .
	manualset3
239753	2	423537	15	NULL	NULL	0	NULL	Gram-negative bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic resistance mechanisms reported in Gram-negative bacteria are causing a worldwide health problem .
	manualset3
239754	3	423537	15	NULL	NULL	0	NULL	health problem	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic resistance mechanisms reported in Gram-negative bacteria are causing a worldwide health problem .
	manualset3
239755	1	423538	15	NULL	NULL	0	NULL	Antibiotic treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic treatment of incipient drug-induced gingival overgrowth in adult renal transplant patients .
	manualset3
239756	2	423538	15	NULL	NULL	0	NULL	drug-induced gingival overgrowth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic treatment of incipient drug-induced gingival overgrowth in adult renal transplant patients .
	manualset3
239757	3	423538	15	NULL	NULL	0	NULL	adult renal transplant patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotic treatment of incipient drug-induced gingival overgrowth in adult renal transplant patients .
	manualset3
239758	1	423539	15	NULL	NULL	0	NULL	Antibiotics 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotics are the primary form of medical treatment for acute bacterial rhinosinusitis , but they should be used when acute bacterial rhinosinusitis presents as persistent or severe disease .
	manualset3
239759	2	423539	15	NULL	NULL	NULL	NULL	primary form of medical treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Antibiotics are the primary form of medical treatment for acute bacterial rhinosinusitis , but they should be used when acute bacterial rhinosinusitis presents as persistent or severe disease .
	manualset3
239760	3	423539	15	NULL	NULL	0	NULL	acute bacterial rhinosinusitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotics are the primary form of medical treatment for acute bacterial rhinosinusitis , but they should be used when acute bacterial rhinosinusitis presents as persistent or severe disease .
	manualset3
239761	4	423539	15	NULL	NULL	0	NULL	acute bacterial rhinosinusitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotics are the primary form of medical treatment for acute bacterial rhinosinusitis , but they should be used when acute bacterial rhinosinusitis presents as persistent or severe disease .
	manualset3
239762	5	423539	15	NULL	NULL	0	NULL	presents	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotics are the primary form of medical treatment for acute bacterial rhinosinusitis , but they should be used when acute bacterial rhinosinusitis presents as persistent or severe disease .
	manualset3
239763	6	423539	15	NULL	NULL	0	NULL	severe disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibiotics are the primary form of medical treatment for acute bacterial rhinosinusitis , but they should be used when acute bacterial rhinosinusitis presents as persistent or severe disease .
	manualset3
239764	1	423540	15	NULL	NULL	0	NULL	Antibodies ( Ab )	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies ( Ab ) specific for canine IL-4 are available from various sources , but these Ab have been produced against recombinant Escherichia coli-expressed canine IL-4 and there is only limited information on their reactivities with native canine IL-4 .
	manualset3
239765	2	423540	15	NULL	NULL	0	NULL	canine IL-4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies ( Ab ) specific for canine IL-4 are available from various sources , but these Ab have been produced against recombinant Escherichia coli-expressed canine IL-4 and there is only limited information on their reactivities with native canine IL-4 .
	manualset3
239766	3	423540	15	NULL	NULL	0	NULL	sources	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies ( Ab ) specific for canine IL-4 are available from various sources , but these Ab have been produced against recombinant Escherichia coli-expressed canine IL-4 and there is only limited information on their reactivities with native canine IL-4 .
	manualset3
239767	4	423540	15	NULL	NULL	0	NULL	 Ab	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies ( Ab ) specific for canine IL-4 are available from various sources , but these Ab have been produced against recombinant Escherichia coli-expressed canine IL-4 and there is only limited information on their reactivities with native canine IL-4 .
	manualset3
239768	5	423540	15	NULL	NULL	0	NULL	recombinant Escherichia coli-expressed canine IL-4 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies ( Ab ) specific for canine IL-4 are available from various sources , but these Ab have been produced against recombinant Escherichia coli-expressed canine IL-4 and there is only limited information on their reactivities with native canine IL-4 .
	manualset3
239769	6	423540	15	NULL	NULL	0	NULL	information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies ( Ab ) specific for canine IL-4 are available from various sources , but these Ab have been produced against recombinant Escherichia coli-expressed canine IL-4 and there is only limited information on their reactivities with native canine IL-4 .
	manualset3
239770	7	423540	15	NULL	NULL	0	NULL	reactivities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies ( Ab ) specific for canine IL-4 are available from various sources , but these Ab have been produced against recombinant Escherichia coli-expressed canine IL-4 and there is only limited information on their reactivities with native canine IL-4 .
	manualset3
239771	8	423540	15	NULL	NULL	0	NULL	 native canine IL-4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies ( Ab ) specific for canine IL-4 are available from various sources , but these Ab have been produced against recombinant Escherichia coli-expressed canine IL-4 and there is only limited information on their reactivities with native canine IL-4 .
	manualset3
239772	1	423541	15	NULL	NULL	0	NULL	Antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies against VCAM-1 and integrin 4 effectively inhibit bone metastasis progression and preserve bone structure .
	manualset3
239773	2	423541	15	NULL	NULL	0	NULL	VCAM-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies against VCAM-1 and integrin 4 effectively inhibit bone metastasis progression and preserve bone structure .
	manualset3
239774	3	423541	15	NULL	NULL	0	NULL	integrin 4 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies against VCAM-1 and integrin 4 effectively inhibit bone metastasis progression and preserve bone structure .
	manualset3
239775	4	423541	15	NULL	NULL	0	NULL	bone metastasis progression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies against VCAM-1 and integrin 4 effectively inhibit bone metastasis progression and preserve bone structure .
	manualset3
239776	5	423541	15	NULL	NULL	0	NULL	bone structure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies against VCAM-1 and integrin 4 effectively inhibit bone metastasis progression and preserve bone structure .
	manualset3
239777	1	423542	15	NULL	NULL	0	NULL	Antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies that are useful in the treatment of HIV infection should result in virus neutralization or lysis of infected cells but should not enhance infection .
	manualset3
239778	2	423542	15	NULL	NULL	0	NULL	treatment of HIV infection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies that are useful in the treatment of HIV infection should result in virus neutralization or lysis of infected cells but should not enhance infection .
	manualset3
239779	3	423542	15	NULL	NULL	0	NULL	result 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies that are useful in the treatment of HIV infection should result in virus neutralization or lysis of infected cells but should not enhance infection .
	manualset3
239780	4	423542	15	NULL	NULL	0	NULL	virus neutralization 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies that are useful in the treatment of HIV infection should result in virus neutralization or lysis of infected cells but should not enhance infection .
	manualset3
239781	5	423542	15	NULL	NULL	NULL	NULL	lysis 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Antibodies that are useful in the treatment of HIV infection should result in virus neutralization or lysis of infected cells but should not enhance infection .
	manualset3
239782	6	423542	15	NULL	NULL	0	NULL	infected cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies that are useful in the treatment of HIV infection should result in virus neutralization or lysis of infected cells but should not enhance infection .
	manualset3
239783	7	423542	15	NULL	NULL	0	NULL	infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies that are useful in the treatment of HIV infection should result in virus neutralization or lysis of infected cells but should not enhance infection .
	manualset3
239786	2	423543	15	NULL	NULL	NULL	NULL	( 2 ) GPI	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Antibodies to ( 2 ) GPI are found in patients with anti-phospholipid syndrome , a systemic autoimmune disease associated with vascular thrombosis and pregnancy morbidity .
	manualset3
239787	3	423543	15	NULL	NULL	NULL	NULL	 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Antibodies to ( 2 ) GPI are found in patients with anti-phospholipid syndrome , a systemic autoimmune disease associated with vascular thrombosis and pregnancy morbidity .
	manualset3
239788	4	423543	15	NULL	NULL	NULL	NULL	anti-phospholipid syndrome 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Antibodies to ( 2 ) GPI are found in patients with anti-phospholipid syndrome , a systemic autoimmune disease associated with vascular thrombosis and pregnancy morbidity .
	manualset3
239789	5	423543	15	NULL	NULL	NULL	NULL	systemic autoimmune disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Antibodies to ( 2 ) GPI are found in patients with anti-phospholipid syndrome , a systemic autoimmune disease associated with vascular thrombosis and pregnancy morbidity .
	manualset3
239790	6	423543	15	NULL	NULL	NULL	NULL	vascular thrombosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Antibodies to ( 2 ) GPI are found in patients with anti-phospholipid syndrome , a systemic autoimmune disease associated with vascular thrombosis and pregnancy morbidity .
	manualset3
239791	7	423543	15	NULL	NULL	NULL	NULL	pregnancy morbidity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Antibodies to ( 2 ) GPI are found in patients with anti-phospholipid syndrome , a systemic autoimmune disease associated with vascular thrombosis and pregnancy morbidity .
	manualset3
239793	1	423543	15	NULL	NULL	0	NULL	Antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies to ( 2 ) GPI are found in patients with anti-phospholipid syndrome , a systemic autoimmune disease associated with vascular thrombosis and pregnancy morbidity .
	manualset3
239795	1	423544	15	NULL	NULL	0	NULL	Antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies to a short synthetic peptide cross-react with human recombinant interleukin 1 alpha .
	manualset3
239796	2	423544	15	NULL	NULL	0	NULL	short synthetic peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies to a short synthetic peptide cross-react with human recombinant interleukin 1 alpha .
	manualset3
239797	3	423544	15	NULL	NULL	0	NULL	human recombinant interleukin 1 alpha 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies to a short synthetic peptide cross-react with human recombinant interleukin 1 alpha .
	manualset3
239798	1	423545	15	NULL	NULL	0	NULL	Antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies to acetylcholine receptor ( AChR ) are major cause of the human autoimmune disease , myasthenia gravis ( MG ) .
	manualset3
239799	2	423545	15	NULL	NULL	0	NULL	acetylcholine receptor ( AChR )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies to acetylcholine receptor ( AChR ) are major cause of the human autoimmune disease , myasthenia gravis ( MG ) .
	manualset3
239800	3	423545	15	NULL	NULL	0	NULL	cause	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies to acetylcholine receptor ( AChR ) are major cause of the human autoimmune disease , myasthenia gravis ( MG ) .
	manualset3
239801	4	423545	15	NULL	NULL	0	NULL	human autoimmune disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies to acetylcholine receptor ( AChR ) are major cause of the human autoimmune disease , myasthenia gravis ( MG ) .
	manualset3
239802	5	423545	15	NULL	NULL	0	NULL	myasthenia gravis ( MG )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibodies to acetylcholine receptor ( AChR ) are major cause of the human autoimmune disease , myasthenia gravis ( MG ) .
	manualset3
239804	1	423546	15	NULL	NULL	0	NULL	Antibody immobilization 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibody immobilization and the hydrophilic properties of the guided-mode resonance filter ( GMRF ) surface were investigated by X-ray photoelectron spectroscopy ( XPS ) and by monitoring the peak wavelength shift and water contact angle ( CA ) .
	manualset3
239806	2	423546	15	NULL	NULL	0	NULL	hydrophilic properties	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibody immobilization and the hydrophilic properties of the guided-mode resonance filter ( GMRF ) surface were investigated by X-ray photoelectron spectroscopy ( XPS ) and by monitoring the peak wavelength shift and water contact angle ( CA ) .
	manualset3
239807	3	423546	15	NULL	NULL	0	NULL	guided-mode resonance filter ( GMRF ) surface	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibody immobilization and the hydrophilic properties of the guided-mode resonance filter ( GMRF ) surface were investigated by X-ray photoelectron spectroscopy ( XPS ) and by monitoring the peak wavelength shift and water contact angle ( CA ) .
	manualset3
239808	4	423546	15	NULL	NULL	0	NULL	X-ray photoelectron spectroscopy ( XPS ) 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibody immobilization and the hydrophilic properties of the guided-mode resonance filter ( GMRF ) surface were investigated by X-ray photoelectron spectroscopy ( XPS ) and by monitoring the peak wavelength shift and water contact angle ( CA ) .
	manualset3
239809	5	423546	15	NULL	NULL	0	NULL	peak wavelength shift	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibody immobilization and the hydrophilic properties of the guided-mode resonance filter ( GMRF ) surface were investigated by X-ray photoelectron spectroscopy ( XPS ) and by monitoring the peak wavelength shift and water contact angle ( CA ) .
	manualset3
239811	6	423546	15	NULL	NULL	0	NULL	water contact angle ( CA )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibody immobilization and the hydrophilic properties of the guided-mode resonance filter ( GMRF ) surface were investigated by X-ray photoelectron spectroscopy ( XPS ) and by monitoring the peak wavelength shift and water contact angle ( CA ) .
	manualset3
239813	1	423547	15	NULL	NULL	0	NULL	Antibody response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibody response of dairy cattle experimentally infected with Listeria monocytogenes .
	manualset3
239814	2	423547	15	NULL	NULL	0	NULL	dairy cattle	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibody response of dairy cattle experimentally infected with Listeria monocytogenes .
	manualset3
239815	3	423547	15	NULL	NULL	0	NULL	Listeria monocytogenes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibody response of dairy cattle experimentally infected with Listeria monocytogenes .
	manualset3
239817	1	423548	15	NULL	NULL	0	NULL	Antibody responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibody responses to SV40 Tag were observed via indirect enzyme-linked immunosorbent assay following three intramuscular ( i.m. ) injections of pCMV-Tag and were typified by a mixed Th1/Th2 response .
	manualset3
239819	2	423548	15	NULL	NULL	0	NULL	SV40 Tag 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibody responses to SV40 Tag were observed via indirect enzyme-linked immunosorbent assay following three intramuscular ( i.m. ) injections of pCMV-Tag and were typified by a mixed Th1/Th2 response .
	manualset3
239821	3	423548	15	NULL	NULL	0	NULL	indirect enzyme-linked immunosorbent assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibody responses to SV40 Tag were observed via indirect enzyme-linked immunosorbent assay following three intramuscular ( i.m. ) injections of pCMV-Tag and were typified by a mixed Th1/Th2 response .
	manualset3
239822	4	423548	15	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibody responses to SV40 Tag were observed via indirect enzyme-linked immunosorbent assay following three intramuscular ( i.m. ) injections of pCMV-Tag and were typified by a mixed Th1/Th2 response .
	manualset3
239823	5	423548	15	NULL	NULL	0	NULL	intramuscular ( i.m. ) injections	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibody responses to SV40 Tag were observed via indirect enzyme-linked immunosorbent assay following three intramuscular ( i.m. ) injections of pCMV-Tag and were typified by a mixed Th1/Th2 response .
	manualset3
239825	6	423548	15	NULL	NULL	0	NULL	pCMV-Tag	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibody responses to SV40 Tag were observed via indirect enzyme-linked immunosorbent assay following three intramuscular ( i.m. ) injections of pCMV-Tag and were typified by a mixed Th1/Th2 response .
	manualset3
239826	7	423548	15	NULL	NULL	0	NULL	mixed Th1/Th2 response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibody responses to SV40 Tag were observed via indirect enzyme-linked immunosorbent assay following three intramuscular ( i.m. ) injections of pCMV-Tag and were typified by a mixed Th1/Th2 response .
	manualset3
239828	1	423549	15	NULL	NULL	0	NULL	Antibody treatments	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibody treatments ( 2.5 mg/kg/day ) given by intraperitoneal injection every 3 days starting 24 h after virus inoculation extended survival time by 1 day relative to placebo-treated animals .
	manualset3
239829	2	423549	15	NULL	NULL	0	NULL	2.5 mg/kg/day	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibody treatments ( 2.5 mg/kg/day ) given by intraperitoneal injection every 3 days starting 24 h after virus inoculation extended survival time by 1 day relative to placebo-treated animals .
	manualset3
239830	3	423549	15	NULL	NULL	0	NULL	intraperitoneal injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Antibody treatments ( 2.5 mg/kg/day ) given by intraperitoneal injection every 3 days starting 24 h after virus inoculation extended survival time by 1 day relative to placebo-treated animals .
	manualset3
239831	4	423549	15	NULL	NULL	NULL	NULL	every 3 days	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Antibody treatments ( 2.5 mg/kg/day ) given by intraperitoneal injection every 3 days starting 24 h after virus inoculation extended survival time by 1 day relative to placebo-treated animals .
	manualset3
239832	5	423549	15	NULL	NULL	NULL	NULL	24 h after virus inoculation 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Antibody treatments ( 2.5 mg/kg/day ) given by intraperitoneal injection every 3 days starting 24 h after virus inoculation extended survival time by 1 day relative to placebo-treated animals .
	manualset3
239834	6	423549	15	NULL	NULL	NULL	NULL	survival time	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Antibody treatments ( 2.5 mg/kg/day ) given by intraperitoneal injection every 3 days starting 24 h after virus inoculation extended survival time by 1 day relative to placebo-treated animals .
	manualset3
239835	7	423549	15	NULL	NULL	NULL	NULL	1 day 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Antibody treatments ( 2.5 mg/kg/day ) given by intraperitoneal injection every 3 days starting 24 h after virus inoculation extended survival time by 1 day relative to placebo-treated animals .
	manualset3
239836	8	423549	15	NULL	NULL	NULL	NULL	placebo-treated animals	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Antibody treatments ( 2.5 mg/kg/day ) given by intraperitoneal injection every 3 days starting 24 h after virus inoculation extended survival time by 1 day relative to placebo-treated animals .
	manualset3
239837	1	423550	15	NULL	NULL	0	NULL	Anticoagulation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Anticoagulation is an important therapeutic strategy to treat and prevent recurrent thrombotic events in patients after acute myocardial infarction and ischemic stroke .
	manualset3
239838	2	423550	15	NULL	NULL	0	NULL	therapeutic strategy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Anticoagulation is an important therapeutic strategy to treat and prevent recurrent thrombotic events in patients after acute myocardial infarction and ischemic stroke .
	manualset3
239839	3	423550	15	NULL	NULL	0	NULL	recurrent thrombotic events	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Anticoagulation is an important therapeutic strategy to treat and prevent recurrent thrombotic events in patients after acute myocardial infarction and ischemic stroke .
	manualset3
239840	4	423550	15	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Anticoagulation is an important therapeutic strategy to treat and prevent recurrent thrombotic events in patients after acute myocardial infarction and ischemic stroke .
	manualset3
239841	5	423550	15	NULL	NULL	0	NULL	acute myocardial infarction	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Anticoagulation is an important therapeutic strategy to treat and prevent recurrent thrombotic events in patients after acute myocardial infarction and ischemic stroke .
	manualset3
239842	6	423550	15	NULL	NULL	0	NULL	ischemic stroke	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Anticoagulation is an important therapeutic strategy to treat and prevent recurrent thrombotic events in patients after acute myocardial infarction and ischemic stroke .
	manualset3
239843	1	423551	15	NULL	NULL	0	NULL	Anticonvulsant drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Anticonvulsant drugs , folate deficiency , and metabolic bone disease .
	manualset3
239844	2	423551	15	NULL	NULL	0	NULL	folate deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Anticonvulsant drugs , folate deficiency , and metabolic bone disease .
	manualset3
239845	3	423551	15	NULL	NULL	0	NULL	metabolic bone disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Anticonvulsant drugs , folate deficiency , and metabolic bone disease .
	manualset3
239846	1	423552	15	NULL	NULL	0	NULL	Anticonvulsant effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Anticonvulsant effects of bilobalide , one of the constituents of Ginkgo biloba L. , on the convulsions induced by 4-O-methylpyridoxine ( MPN ) were investigated in mice .
	manualset3
239847	2	423552	15	NULL	NULL	0	NULL	bilobalide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Anticonvulsant effects of bilobalide , one of the constituents of Ginkgo biloba L. , on the convulsions induced by 4-O-methylpyridoxine ( MPN ) were investigated in mice .
	manualset3
239848	3	423552	15	NULL	NULL	0	NULL	constituents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Anticonvulsant effects of bilobalide , one of the constituents of Ginkgo biloba L. , on the convulsions induced by 4-O-methylpyridoxine ( MPN ) were investigated in mice .
	manualset3
239849	4	423552	15	NULL	NULL	0	NULL	Ginkgo biloba L	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Anticonvulsant effects of bilobalide , one of the constituents of Ginkgo biloba L. , on the convulsions induced by 4-O-methylpyridoxine ( MPN ) were investigated in mice .
	manualset3
239850	5	423552	15	NULL	NULL	0	NULL	convulsions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Anticonvulsant effects of bilobalide , one of the constituents of Ginkgo biloba L. , on the convulsions induced by 4-O-methylpyridoxine ( MPN ) were investigated in mice .
	manualset3
239851	6	423552	15	NULL	NULL	0	NULL	4-O-methylpyridoxine ( MPN )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Anticonvulsant effects of bilobalide , one of the constituents of Ginkgo biloba L. , on the convulsions induced by 4-O-methylpyridoxine ( MPN ) were investigated in mice .
	manualset3
239852	7	423552	15	NULL	NULL	0	NULL	 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Anticonvulsant effects of bilobalide , one of the constituents of Ginkgo biloba L. , on the convulsions induced by 4-O-methylpyridoxine ( MPN ) were investigated in mice .
	manualset3
239853	1	423553	15	NULL	NULL	0	NULL	Antidepressant-like effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antidepressant-like effect of tramadol in the unpredictable chronic mild stress procedure : possible involvement of the noradrenergic system .
	manualset3
239854	2	423553	15	NULL	NULL	0	NULL	tramadol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Antidepressant-like effect of tramadol in the unpredictable chronic mild stress procedure : possible involvement of the noradrenergic system .
	manualset3
239855	3	423553	15	NULL	NULL	0	NULL	chronic mild stress procedure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antidepressant-like effect of tramadol in the unpredictable chronic mild stress procedure : possible involvement of the noradrenergic system .
	manualset3
239856	4	423553	15	NULL	NULL	0	NULL	involvement of the noradrenergic system 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antidepressant-like effect of tramadol in the unpredictable chronic mild stress procedure : possible involvement of the noradrenergic system .
	manualset3
239857	1	423554	15	NULL	NULL	0	NULL	Antidepressant-like effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antidepressant-like effects of CCK ( B ) receptor antagonists : involvement of the opioid system .
	manualset3
239858	2	423554	15	NULL	NULL	0	NULL	CCK ( B ) receptor antagonists	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Antidepressant-like effects of CCK ( B ) receptor antagonists : involvement of the opioid system .
	manualset3
239859	3	423554	15	NULL	NULL	0	NULL	involvement of the opioid system	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antidepressant-like effects of CCK ( B ) receptor antagonists : involvement of the opioid system .
	manualset3
239860	1	423555	15	NULL	NULL	0	NULL	Antidepressant clinical trials	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Antidepressant clinical trials and subject recruitment : just who are symptomatic volunteers ?
	manualset3
239861	2	423555	15	NULL	NULL	0	NULL	subject recruitment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Antidepressant clinical trials and subject recruitment : just who are symptomatic volunteers ?
	manualset3
239862	3	423555	15	NULL	NULL	0	NULL	symptomatic volunteers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Antidepressant clinical trials and subject recruitment : just who are symptomatic volunteers ?
	manualset3
239863	1	423556	15	NULL	NULL	0	NULL	EXPERIENCES	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( EXPERIENCES FROM WORK OF IMPROVING SANITARY EDUCATION ON DAIRY FARMS ) .
	manualset3
239865	2	423556	15	NULL	NULL	0	NULL	WORK OF IMPROVING SANITARY EDUCATION	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( EXPERIENCES FROM WORK OF IMPROVING SANITARY EDUCATION ON DAIRY FARMS ) .
	manualset3
239866	3	423556	15	NULL	NULL	0	NULL	DAIRY FARMS	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( EXPERIENCES FROM WORK OF IMPROVING SANITARY EDUCATION ON DAIRY FARMS ) .
	manualset3
239867	1	423557	15	NULL	NULL	0	NULL	Antidepressant use 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Antidepressant use did not vary by race/ethnicity .
	manualset3
239869	2	423557	15	NULL	NULL	0	NULL	race	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Antidepressant use did not vary by race/ethnicity .
	manualset3
239870	3	423557	15	NULL	NULL	0	NULL	ethnicity	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Antidepressant use did not vary by race/ethnicity .
	manualset3
239871	1	423558	15	NULL	NULL	0	NULL	Antidiabetic screening	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Antidiabetic screening of commercial botanical products in 3T3-L1 adipocytes and db/db mice .
	manualset3
239872	2	423558	15	NULL	NULL	0	NULL	commercial botanical products	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Antidiabetic screening of commercial botanical products in 3T3-L1 adipocytes and db/db mice .
	manualset3
239873	3	423558	15	NULL	NULL	0	NULL	3T3-L1 adipocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Antidiabetic screening of commercial botanical products in 3T3-L1 adipocytes and db/db mice .
	manualset3
239874	4	423558	15	NULL	NULL	0	NULL	db/db mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Antidiabetic screening of commercial botanical products in 3T3-L1 adipocytes and db/db mice .
	manualset3
239875	1	423559	15	NULL	NULL	0	NULL	Antifolate antimalarial drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Antifolate antimalarial drugs interfere with folate metabolism , a pathway essential to malaria parasite survival .
	manualset3
239876	2	423559	15	NULL	NULL	0	NULL	folate metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antifolate antimalarial drugs interfere with folate metabolism , a pathway essential to malaria parasite survival .
	manualset3
239877	3	423559	15	NULL	NULL	0	NULL	pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antifolate antimalarial drugs interfere with folate metabolism , a pathway essential to malaria parasite survival .
	manualset3
239878	4	423559	15	NULL	NULL	0	NULL	malaria parasite survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antifolate antimalarial drugs interfere with folate metabolism , a pathway essential to malaria parasite survival .
	manualset3
239879	1	423560	15	NULL	NULL	0	NULL	Antigen	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Antigen endocytosed via CD205 enters the MHC class I and MHC class II antigen presentation pathways and is subsequently presented to both CD4 + and CD8 + T cells .
	manualset3
239880	2	423560	15	NULL	NULL	0	NULL	CD205	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Antigen endocytosed via CD205 enters the MHC class I and MHC class II antigen presentation pathways and is subsequently presented to both CD4 + and CD8 + T cells .
	manualset3
239881	3	423560	15	NULL	NULL	0	NULL	MHC class I antigen presentation pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antigen endocytosed via CD205 enters the MHC class I and MHC class II antigen presentation pathways and is subsequently presented to both CD4 + and CD8 + T cells .
	manualset3
239882	4	423560	15	NULL	NULL	0	NULL	MHC class II antigen presentation pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antigen endocytosed via CD205 enters the MHC class I and MHC class II antigen presentation pathways and is subsequently presented to both CD4 + and CD8 + T cells .
	manualset3
239883	5	423560	15	NULL	NULL	0	NULL	CD4 + T cells . 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Antigen endocytosed via CD205 enters the MHC class I and MHC class II antigen presentation pathways and is subsequently presented to both CD4 + and CD8 + T cells .
	manualset3
239884	6	423560	15	NULL	NULL	0	NULL	CD8 + T cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Antigen endocytosed via CD205 enters the MHC class I and MHC class II antigen presentation pathways and is subsequently presented to both CD4 + and CD8 + T cells .
	manualset3
239885	1	423561	15	NULL	NULL	0	NULL	Antigen presentation events 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antigen presentation events in autoimmune diabetes .
	manualset3
239886	2	423561	15	NULL	NULL	0	NULL	autoimmune diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Antigen presentation events in autoimmune diabetes .
	manualset3
239887	1	423562	15	NULL	NULL	0	NULL	Antigenic diversity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antigenic diversity of Ehrlichia chaffeensis and Ehrlichia canis may involve independent or differential expression of the P28 outer membrane proteins genes , enabling persistent infections of the natural hosts .
	manualset3
239888	2	423562	15	NULL	NULL	0	NULL	Ehrlichia chaffeensis 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Antigenic diversity of Ehrlichia chaffeensis and Ehrlichia canis may involve independent or differential expression of the P28 outer membrane proteins genes , enabling persistent infections of the natural hosts .
	manualset3
239889	3	423562	15	NULL	NULL	0	NULL	Ehrlichia canis 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Antigenic diversity of Ehrlichia chaffeensis and Ehrlichia canis may involve independent or differential expression of the P28 outer membrane proteins genes , enabling persistent infections of the natural hosts .
	manualset3
239891	4	423562	15	NULL	NULL	0	NULL	independent expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antigenic diversity of Ehrlichia chaffeensis and Ehrlichia canis may involve independent or differential expression of the P28 outer membrane proteins genes , enabling persistent infections of the natural hosts .
	manualset3
239893	5	423562	15	NULL	NULL	0	NULL	differential expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antigenic diversity of Ehrlichia chaffeensis and Ehrlichia canis may involve independent or differential expression of the P28 outer membrane proteins genes , enabling persistent infections of the natural hosts .
	manualset3
239894	6	423562	15	NULL	NULL	0	NULL	P28 outer membrane proteins genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Antigenic diversity of Ehrlichia chaffeensis and Ehrlichia canis may involve independent or differential expression of the P28 outer membrane proteins genes , enabling persistent infections of the natural hosts .
	manualset3
239895	7	423562	15	NULL	NULL	0	NULL	persistent infections 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antigenic diversity of Ehrlichia chaffeensis and Ehrlichia canis may involve independent or differential expression of the P28 outer membrane proteins genes , enabling persistent infections of the natural hosts .
	manualset3
239896	8	423562	15	NULL	NULL	0	NULL	natural hosts	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Antigenic diversity of Ehrlichia chaffeensis and Ehrlichia canis may involve independent or differential expression of the P28 outer membrane proteins genes , enabling persistent infections of the natural hosts .
	manualset3
239897	1	423563	15	NULL	NULL	0	NULL	EXPERIMENTAL STUDY	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( EXPERIMENTAL STUDY ON THE PROBLEM OF THE SIGNIFICANCE OF INTRAVASCULAR FIBRIN FORMATION IN THE OCCURRANCE OF ARTERIOSCLEROTIC CHANGES IN THE WALLS OF BLOOD VESSELS ) .
	manualset3
239898	2	423563	15	NULL	NULL	NULL	NULL	PROBLEM OF THE SIGNIFICANCE	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( EXPERIMENTAL STUDY ON THE PROBLEM OF THE SIGNIFICANCE OF INTRAVASCULAR FIBRIN FORMATION IN THE OCCURRANCE OF ARTERIOSCLEROTIC CHANGES IN THE WALLS OF BLOOD VESSELS ) .
	manualset3
239899	3	423563	15	NULL	NULL	0	NULL	INTRAVASCULAR FIBRIN FORMATION	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( EXPERIMENTAL STUDY ON THE PROBLEM OF THE SIGNIFICANCE OF INTRAVASCULAR FIBRIN FORMATION IN THE OCCURRANCE OF ARTERIOSCLEROTIC CHANGES IN THE WALLS OF BLOOD VESSELS ) .
	manualset3
239900	4	423563	15	NULL	NULL	0	NULL	OCCURRANCE 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( EXPERIMENTAL STUDY ON THE PROBLEM OF THE SIGNIFICANCE OF INTRAVASCULAR FIBRIN FORMATION IN THE OCCURRANCE OF ARTERIOSCLEROTIC CHANGES IN THE WALLS OF BLOOD VESSELS ) .
	manualset3
239901	5	423563	15	NULL	NULL	0	NULL	ARTERIOSCLEROTIC CHANGES	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( EXPERIMENTAL STUDY ON THE PROBLEM OF THE SIGNIFICANCE OF INTRAVASCULAR FIBRIN FORMATION IN THE OCCURRANCE OF ARTERIOSCLEROTIC CHANGES IN THE WALLS OF BLOOD VESSELS ) .
	manualset3
239902	6	423563	15	NULL	NULL	0	NULL	WALLS OF BLOOD VESSELS	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( EXPERIMENTAL STUDY ON THE PROBLEM OF THE SIGNIFICANCE OF INTRAVASCULAR FIBRIN FORMATION IN THE OCCURRANCE OF ARTERIOSCLEROTIC CHANGES IN THE WALLS OF BLOOD VESSELS ) .
	manualset3
239903	1	423564	15	NULL	NULL	0	NULL	Antigenic modulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antigenic modulation and rituximab resistance .
	manualset3
239904	2	423564	15	NULL	NULL	0	NULL	rituximab resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antigenic modulation and rituximab resistance .
	manualset3
239906	1	423565	15	NULL	NULL	0	NULL	Antigens	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Antigens prepared from each of five strains ( CA , CJ , HB-1 , HB-3 , and TY ) of pathogenic Naegleria and the EG strain of nonpathogenic Naegleria gruberi were compared by the gel diffusion and immunoelectrophoresis techniques .
	manualset3
239907	2	423565	15	NULL	NULL	0	NULL	five	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Antigens prepared from each of five strains ( CA , CJ , HB-1 , HB-3 , and TY ) of pathogenic Naegleria and the EG strain of nonpathogenic Naegleria gruberi were compared by the gel diffusion and immunoelectrophoresis techniques .
	manualset3
239908	3	423565	15	NULL	NULL	0	NULL	strain CA	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Antigens prepared from each of five strains ( CA , CJ , HB-1 , HB-3 , and TY ) of pathogenic Naegleria and the EG strain of nonpathogenic Naegleria gruberi were compared by the gel diffusion and immunoelectrophoresis techniques .
	manualset3
239909	4	423565	15	NULL	NULL	0	NULL	strain CJ	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Antigens prepared from each of five strains ( CA , CJ , HB-1 , HB-3 , and TY ) of pathogenic Naegleria and the EG strain of nonpathogenic Naegleria gruberi were compared by the gel diffusion and immunoelectrophoresis techniques .
	manualset3
239910	5	423565	15	NULL	NULL	0	NULL	strains HB-1 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Antigens prepared from each of five strains ( CA , CJ , HB-1 , HB-3 , and TY ) of pathogenic Naegleria and the EG strain of nonpathogenic Naegleria gruberi were compared by the gel diffusion and immunoelectrophoresis techniques .
	manualset3
239911	6	423565	15	NULL	NULL	0	NULL	strains HB-3	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Antigens prepared from each of five strains ( CA , CJ , HB-1 , HB-3 , and TY ) of pathogenic Naegleria and the EG strain of nonpathogenic Naegleria gruberi were compared by the gel diffusion and immunoelectrophoresis techniques .
	manualset3
239912	7	423565	15	NULL	NULL	0	NULL	strain TY	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Antigens prepared from each of five strains ( CA , CJ , HB-1 , HB-3 , and TY ) of pathogenic Naegleria and the EG strain of nonpathogenic Naegleria gruberi were compared by the gel diffusion and immunoelectrophoresis techniques .
	manualset3
239913	8	423565	15	NULL	NULL	0	NULL	pathogenic Naegleria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Antigens prepared from each of five strains ( CA , CJ , HB-1 , HB-3 , and TY ) of pathogenic Naegleria and the EG strain of nonpathogenic Naegleria gruberi were compared by the gel diffusion and immunoelectrophoresis techniques .
	manualset3
239914	9	423565	15	NULL	NULL	0	NULL	EG strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Antigens prepared from each of five strains ( CA , CJ , HB-1 , HB-3 , and TY ) of pathogenic Naegleria and the EG strain of nonpathogenic Naegleria gruberi were compared by the gel diffusion and immunoelectrophoresis techniques .
	manualset3
239915	10	423565	15	NULL	NULL	0	NULL	nonpathogenic Naegleria gruberi 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Antigens prepared from each of five strains ( CA , CJ , HB-1 , HB-3 , and TY ) of pathogenic Naegleria and the EG strain of nonpathogenic Naegleria gruberi were compared by the gel diffusion and immunoelectrophoresis techniques .
	manualset3
239916	11	423565	15	NULL	NULL	0	NULL	 gel diffusion techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Antigens prepared from each of five strains ( CA , CJ , HB-1 , HB-3 , and TY ) of pathogenic Naegleria and the EG strain of nonpathogenic Naegleria gruberi were compared by the gel diffusion and immunoelectrophoresis techniques .
	manualset3
239917	12	423565	15	NULL	NULL	0	NULL	immunoelectrophoresis techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Antigens prepared from each of five strains ( CA , CJ , HB-1 , HB-3 , and TY ) of pathogenic Naegleria and the EG strain of nonpathogenic Naegleria gruberi were compared by the gel diffusion and immunoelectrophoresis techniques .
	manualset3
239918	1	423566	15	NULL	NULL	0	NULL	Antihypertensive activity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antihypertensive activity of carvedilol ( 5 mg ) was sufficient in only three cases , but after 4 weeks ( inpatients ) or 8 weeks ( outpatients ) administration of carvedilol ( 10 mg or 20 mg ) , DBP/systolic blood pressure was significantly reduced from 176 + / - 6/117 + / - 3 to 145 + / - 3/94 + / - 2 mm Hg ( p less than 0.001 ) in all patients .
	manualset3
239919	2	423566	15	NULL	NULL	0	NULL	carvedilol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Antihypertensive activity of carvedilol ( 5 mg ) was sufficient in only three cases , but after 4 weeks ( inpatients ) or 8 weeks ( outpatients ) administration of carvedilol ( 10 mg or 20 mg ) , DBP/systolic blood pressure was significantly reduced from 176 + / - 6/117 + / - 3 to 145 + / - 3/94 + / - 2 mm Hg ( p less than 0.001 ) in all patients .
	manualset3
239920	3	423566	15	NULL	NULL	0	NULL	5 mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Antihypertensive activity of carvedilol ( 5 mg ) was sufficient in only three cases , but after 4 weeks ( inpatients ) or 8 weeks ( outpatients ) administration of carvedilol ( 10 mg or 20 mg ) , DBP/systolic blood pressure was significantly reduced from 176 + / - 6/117 + / - 3 to 145 + / - 3/94 + / - 2 mm Hg ( p less than 0.001 ) in all patients .
	manualset3
239921	4	423566	15	NULL	NULL	0	NULL	three cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Antihypertensive activity of carvedilol ( 5 mg ) was sufficient in only three cases , but after 4 weeks ( inpatients ) or 8 weeks ( outpatients ) administration of carvedilol ( 10 mg or 20 mg ) , DBP/systolic blood pressure was significantly reduced from 176 + / - 6/117 + / - 3 to 145 + / - 3/94 + / - 2 mm Hg ( p less than 0.001 ) in all patients .
	manualset3
239922	5	423566	15	NULL	NULL	0	NULL	4 weeks 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Antihypertensive activity of carvedilol ( 5 mg ) was sufficient in only three cases , but after 4 weeks ( inpatients ) or 8 weeks ( outpatients ) administration of carvedilol ( 10 mg or 20 mg ) , DBP/systolic blood pressure was significantly reduced from 176 + / - 6/117 + / - 3 to 145 + / - 3/94 + / - 2 mm Hg ( p less than 0.001 ) in all patients .
	manualset3
239923	6	423566	15	NULL	NULL	0	NULL	inpatients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Antihypertensive activity of carvedilol ( 5 mg ) was sufficient in only three cases , but after 4 weeks ( inpatients ) or 8 weeks ( outpatients ) administration of carvedilol ( 10 mg or 20 mg ) , DBP/systolic blood pressure was significantly reduced from 176 + / - 6/117 + / - 3 to 145 + / - 3/94 + / - 2 mm Hg ( p less than 0.001 ) in all patients .
	manualset3
239924	7	423566	15	NULL	NULL	0	NULL	8 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Antihypertensive activity of carvedilol ( 5 mg ) was sufficient in only three cases , but after 4 weeks ( inpatients ) or 8 weeks ( outpatients ) administration of carvedilol ( 10 mg or 20 mg ) , DBP/systolic blood pressure was significantly reduced from 176 + / - 6/117 + / - 3 to 145 + / - 3/94 + / - 2 mm Hg ( p less than 0.001 ) in all patients .
	manualset3
239925	8	423566	15	NULL	NULL	0	NULL	outpatients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Antihypertensive activity of carvedilol ( 5 mg ) was sufficient in only three cases , but after 4 weeks ( inpatients ) or 8 weeks ( outpatients ) administration of carvedilol ( 10 mg or 20 mg ) , DBP/systolic blood pressure was significantly reduced from 176 + / - 6/117 + / - 3 to 145 + / - 3/94 + / - 2 mm Hg ( p less than 0.001 ) in all patients .
	manualset3
239926	9	423566	15	NULL	NULL	0	NULL	administration of carvedilol 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Antihypertensive activity of carvedilol ( 5 mg ) was sufficient in only three cases , but after 4 weeks ( inpatients ) or 8 weeks ( outpatients ) administration of carvedilol ( 10 mg or 20 mg ) , DBP/systolic blood pressure was significantly reduced from 176 + / - 6/117 + / - 3 to 145 + / - 3/94 + / - 2 mm Hg ( p less than 0.001 ) in all patients .
	manualset3
239927	10	423566	15	NULL	NULL	0	NULL	10 mg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Antihypertensive activity of carvedilol ( 5 mg ) was sufficient in only three cases , but after 4 weeks ( inpatients ) or 8 weeks ( outpatients ) administration of carvedilol ( 10 mg or 20 mg ) , DBP/systolic blood pressure was significantly reduced from 176 + / - 6/117 + / - 3 to 145 + / - 3/94 + / - 2 mm Hg ( p less than 0.001 ) in all patients .
	manualset3
239928	11	423566	15	NULL	NULL	0	NULL	20 mg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Antihypertensive activity of carvedilol ( 5 mg ) was sufficient in only three cases , but after 4 weeks ( inpatients ) or 8 weeks ( outpatients ) administration of carvedilol ( 10 mg or 20 mg ) , DBP/systolic blood pressure was significantly reduced from 176 + / - 6/117 + / - 3 to 145 + / - 3/94 + / - 2 mm Hg ( p less than 0.001 ) in all patients .
	manualset3
239929	12	423566	15	NULL	NULL	0	NULL	DBP/systolic blood pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antihypertensive activity of carvedilol ( 5 mg ) was sufficient in only three cases , but after 4 weeks ( inpatients ) or 8 weeks ( outpatients ) administration of carvedilol ( 10 mg or 20 mg ) , DBP/systolic blood pressure was significantly reduced from 176 + / - 6/117 + / - 3 to 145 + / - 3/94 + / - 2 mm Hg ( p less than 0.001 ) in all patients .
	manualset3
239930	13	423566	15	NULL	NULL	NULL	NULL	176 + / - 6/117 + / - 3 mm Hg 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Antihypertensive activity of carvedilol ( 5 mg ) was sufficient in only three cases , but after 4 weeks ( inpatients ) or 8 weeks ( outpatients ) administration of carvedilol ( 10 mg or 20 mg ) , DBP/systolic blood pressure was significantly reduced from 176 + / - 6/117 + / - 3 to 145 + / - 3/94 + / - 2 mm Hg ( p less than 0.001 ) in all patients .
	manualset3
239931	14	423566	15	NULL	NULL	0	NULL	145 + / - 3/94 + / - 2 mm Hg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Antihypertensive activity of carvedilol ( 5 mg ) was sufficient in only three cases , but after 4 weeks ( inpatients ) or 8 weeks ( outpatients ) administration of carvedilol ( 10 mg or 20 mg ) , DBP/systolic blood pressure was significantly reduced from 176 + / - 6/117 + / - 3 to 145 + / - 3/94 + / - 2 mm Hg ( p less than 0.001 ) in all patients .
	manualset3
239932	15	423566	15	NULL	NULL	0	NULL	 p less than 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Antihypertensive activity of carvedilol ( 5 mg ) was sufficient in only three cases , but after 4 weeks ( inpatients ) or 8 weeks ( outpatients ) administration of carvedilol ( 10 mg or 20 mg ) , DBP/systolic blood pressure was significantly reduced from 176 + / - 6/117 + / - 3 to 145 + / - 3/94 + / - 2 mm Hg ( p less than 0.001 ) in all patients .
	manualset3
239933	16	423566	15	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Antihypertensive activity of carvedilol ( 5 mg ) was sufficient in only three cases , but after 4 weeks ( inpatients ) or 8 weeks ( outpatients ) administration of carvedilol ( 10 mg or 20 mg ) , DBP/systolic blood pressure was significantly reduced from 176 + / - 6/117 + / - 3 to 145 + / - 3/94 + / - 2 mm Hg ( p less than 0.001 ) in all patients .
	manualset3
239934	1	423567	15	NULL	NULL	0	NULL	Antimalarial agents	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Antimalarial agents ameliorate disease in more than half of patients with cutaneous lupus erythematosus ( CLE ) , regardless of smoking status .
	manualset3
239935	2	423567	15	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Antimalarial agents ameliorate disease in more than half of patients with cutaneous lupus erythematosus ( CLE ) , regardless of smoking status .
	manualset3
239936	3	423567	15	NULL	NULL	0	NULL	more than half 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Antimalarial agents ameliorate disease in more than half of patients with cutaneous lupus erythematosus ( CLE ) , regardless of smoking status .
	manualset3
239937	4	423567	15	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Antimalarial agents ameliorate disease in more than half of patients with cutaneous lupus erythematosus ( CLE ) , regardless of smoking status .
	manualset3
239938	5	423567	15	NULL	NULL	0	NULL	cutaneous lupus erythematosus ( CLE )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Antimalarial agents ameliorate disease in more than half of patients with cutaneous lupus erythematosus ( CLE ) , regardless of smoking status .
	manualset3
239939	6	423567	15	NULL	NULL	0	NULL	smoking status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antimalarial agents ameliorate disease in more than half of patients with cutaneous lupus erythematosus ( CLE ) , regardless of smoking status .
	manualset3
239943	1	423568	15	NULL	NULL	0	NULL	Antimicrobial agents	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Antimicrobial agents are used to combat infections ; however breakpoints for M. hyosynoviae have not yet been established .
	manualset3
239944	2	423568	15	NULL	NULL	0	NULL	 infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antimicrobial agents are used to combat infections ; however breakpoints for M. hyosynoviae have not yet been established .
	manualset3
239945	3	423568	15	NULL	NULL	0	NULL	breakpoints	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Antimicrobial agents are used to combat infections ; however breakpoints for M. hyosynoviae have not yet been established .
	manualset3
239946	4	423568	15	NULL	NULL	0	NULL	M. hyosynoviae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Antimicrobial agents are used to combat infections ; however breakpoints for M. hyosynoviae have not yet been established .
	manualset3
239947	1	423569	15	NULL	NULL	0	NULL	Antimicrobial chitosan-lysozyme ( CL ) films	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Antimicrobial chitosan-lysozyme ( CL ) films and coatings for enhancing microbial safety of mozzarella cheese .
	manualset3
239948	2	423569	15	NULL	NULL	0	NULL	Antimicrobial chitosan-lysozyme ( CL ) coatings 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Antimicrobial chitosan-lysozyme ( CL ) films and coatings for enhancing microbial safety of mozzarella cheese .
	manualset3
239949	3	423569	15	NULL	NULL	NULL	NULL	enhancing microbial safety 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Antimicrobial chitosan-lysozyme ( CL ) films and coatings for enhancing microbial safety of mozzarella cheese .
	manualset3
239950	4	423569	15	NULL	NULL	0	NULL	mozzarella cheese	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Antimicrobial chitosan-lysozyme ( CL ) films and coatings for enhancing microbial safety of mozzarella cheese .
	manualset3
239951	1	423570	15	NULL	NULL	0	NULL	Antimuscarinic agents	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Antimuscarinic agents are the most widely used therapy for urge incontinence , but have side effects such as constipation , tachycardia and dry mouth , resulting from a lack of selectivity for the bladder .
	manualset3
239952	2	423570	15	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Antimuscarinic agents are the most widely used therapy for urge incontinence , but have side effects such as constipation , tachycardia and dry mouth , resulting from a lack of selectivity for the bladder .
	manualset3
239953	3	423570	15	NULL	NULL	0	NULL	urge incontinence	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antimuscarinic agents are the most widely used therapy for urge incontinence , but have side effects such as constipation , tachycardia and dry mouth , resulting from a lack of selectivity for the bladder .
	manualset3
239954	4	423570	15	NULL	NULL	0	NULL	side effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antimuscarinic agents are the most widely used therapy for urge incontinence , but have side effects such as constipation , tachycardia and dry mouth , resulting from a lack of selectivity for the bladder .
	manualset3
239955	5	423570	15	NULL	NULL	0	NULL	constipation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antimuscarinic agents are the most widely used therapy for urge incontinence , but have side effects such as constipation , tachycardia and dry mouth , resulting from a lack of selectivity for the bladder .
	manualset3
239957	6	423570	15	NULL	NULL	0	NULL	tachycardia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antimuscarinic agents are the most widely used therapy for urge incontinence , but have side effects such as constipation , tachycardia and dry mouth , resulting from a lack of selectivity for the bladder .
	manualset3
239958	7	423570	15	NULL	NULL	0	NULL	dry mouth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antimuscarinic agents are the most widely used therapy for urge incontinence , but have side effects such as constipation , tachycardia and dry mouth , resulting from a lack of selectivity for the bladder .
	manualset3
239959	8	423570	15	NULL	NULL	0	NULL	lack of selectivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antimuscarinic agents are the most widely used therapy for urge incontinence , but have side effects such as constipation , tachycardia and dry mouth , resulting from a lack of selectivity for the bladder .
	manualset3
239960	9	423570	15	NULL	NULL	0	NULL	bladder	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Antimuscarinic agents are the most widely used therapy for urge incontinence , but have side effects such as constipation , tachycardia and dry mouth , resulting from a lack of selectivity for the bladder .
	manualset3
239961	1	423571	15	NULL	NULL	0	NULL	Early signs of occupational ototoxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Early signs of occupational ototoxicity caused by inhalation of benzene derivative industrial solvents ) .
	manualset3
240234	2	423571	15	NULL	NULL	0	NULL	inhalation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Early signs of occupational ototoxicity caused by inhalation of benzene derivative industrial solvents ) .
	manualset3
240235	3	423571	15	NULL	NULL	0	NULL	benzene derivative industrial solvents 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Early signs of occupational ototoxicity caused by inhalation of benzene derivative industrial solvents ) .
	manualset3
240236	1	423572	15	NULL	NULL	0	NULL	Antiphospholipid syndrome ( APLS )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Antiphospholipid syndrome ( APLS ) is characterized by recurrent thromboembolic phenomena , thrombocytopenia and fetal loss .
	manualset3
240237	2	423572	15	NULL	NULL	0	NULL	recurrent thromboembolic phenomena	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antiphospholipid syndrome ( APLS ) is characterized by recurrent thromboembolic phenomena , thrombocytopenia and fetal loss .
	manualset3
240238	3	423572	15	NULL	NULL	0	NULL	 thrombocytopenia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antiphospholipid syndrome ( APLS ) is characterized by recurrent thromboembolic phenomena , thrombocytopenia and fetal loss .
	manualset3
240239	4	423572	15	NULL	NULL	0	NULL	fetal loss	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antiphospholipid syndrome ( APLS ) is characterized by recurrent thromboembolic phenomena , thrombocytopenia and fetal loss .
	manualset3
240240	1	423573	15	NULL	NULL	0	NULL	Antipyrine metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antipyrine metabolism , therefore , depends on the severity rather than the etiology of liver disease and may serve as a measure of hepatic function irrespective of the cause of liver disease .
	manualset3
240241	2	423573	15	NULL	NULL	NULL	NULL	severity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Antipyrine metabolism , therefore , depends on the severity rather than the etiology of liver disease and may serve as a measure of hepatic function irrespective of the cause of liver disease .
	manualset3
240242	3	423573	15	NULL	NULL	0	NULL	etiology of liver disease	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antipyrine metabolism , therefore , depends on the severity rather than the etiology of liver disease and may serve as a measure of hepatic function irrespective of the cause of liver disease .
	manualset3
240243	4	423573	15	NULL	NULL	0	NULL	measure of hepatic function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antipyrine metabolism , therefore , depends on the severity rather than the etiology of liver disease and may serve as a measure of hepatic function irrespective of the cause of liver disease .
	manualset3
240244	5	423573	15	NULL	NULL	0	NULL	cause of liver disease	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antipyrine metabolism , therefore , depends on the severity rather than the etiology of liver disease and may serve as a measure of hepatic function irrespective of the cause of liver disease .
	manualset3
240245	1	423574	15	NULL	NULL	0	NULL	Antiretroviral monotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Antiretroviral monotherapy and combination therapy is widely prescribed in pregnancy because : ( i ) with appropriate management , which includes antiretroviral therapy , the risk of mother-to-child transmission can be reduced from 15 to 25 % to less than 1 % ; ( ii ) pregnant women with advanced HIV infection require therapy ; ( iii ) combination therapy with at least 3 compounds significantly reduces morbidity and mortality compared with dual or monotherapy ; and ( iv ) the benefits of therapy for both the mother and the infant outweigh the risk .
	manualset3
240246	2	423574	15	NULL	NULL	0	NULL	combination therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Antiretroviral monotherapy and combination therapy is widely prescribed in pregnancy because : ( i ) with appropriate management , which includes antiretroviral therapy , the risk of mother-to-child transmission can be reduced from 15 to 25 % to less than 1 % ; ( ii ) pregnant women with advanced HIV infection require therapy ; ( iii ) combination therapy with at least 3 compounds significantly reduces morbidity and mortality compared with dual or monotherapy ; and ( iv ) the benefits of therapy for both the mother and the infant outweigh the risk .
	manualset3
240247	3	423574	15	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antiretroviral monotherapy and combination therapy is widely prescribed in pregnancy because : ( i ) with appropriate management , which includes antiretroviral therapy , the risk of mother-to-child transmission can be reduced from 15 to 25 % to less than 1 % ; ( ii ) pregnant women with advanced HIV infection require therapy ; ( iii ) combination therapy with at least 3 compounds significantly reduces morbidity and mortality compared with dual or monotherapy ; and ( iv ) the benefits of therapy for both the mother and the infant outweigh the risk .
	manualset3
240248	4	423574	15	NULL	NULL	0	NULL	appropriate management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Antiretroviral monotherapy and combination therapy is widely prescribed in pregnancy because : ( i ) with appropriate management , which includes antiretroviral therapy , the risk of mother-to-child transmission can be reduced from 15 to 25 % to less than 1 % ; ( ii ) pregnant women with advanced HIV infection require therapy ; ( iii ) combination therapy with at least 3 compounds significantly reduces morbidity and mortality compared with dual or monotherapy ; and ( iv ) the benefits of therapy for both the mother and the infant outweigh the risk .
	manualset3
240249	5	423574	15	NULL	NULL	0	NULL	antiretroviral therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Antiretroviral monotherapy and combination therapy is widely prescribed in pregnancy because : ( i ) with appropriate management , which includes antiretroviral therapy , the risk of mother-to-child transmission can be reduced from 15 to 25 % to less than 1 % ; ( ii ) pregnant women with advanced HIV infection require therapy ; ( iii ) combination therapy with at least 3 compounds significantly reduces morbidity and mortality compared with dual or monotherapy ; and ( iv ) the benefits of therapy for both the mother and the infant outweigh the risk .
	manualset3
240250	6	423574	15	NULL	NULL	0	NULL	risk of mother-to-child transmission	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antiretroviral monotherapy and combination therapy is widely prescribed in pregnancy because : ( i ) with appropriate management , which includes antiretroviral therapy , the risk of mother-to-child transmission can be reduced from 15 to 25 % to less than 1 % ; ( ii ) pregnant women with advanced HIV infection require therapy ; ( iii ) combination therapy with at least 3 compounds significantly reduces morbidity and mortality compared with dual or monotherapy ; and ( iv ) the benefits of therapy for both the mother and the infant outweigh the risk .
	manualset3
240251	7	423574	15	NULL	NULL	0	NULL	15 to 25 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Antiretroviral monotherapy and combination therapy is widely prescribed in pregnancy because : ( i ) with appropriate management , which includes antiretroviral therapy , the risk of mother-to-child transmission can be reduced from 15 to 25 % to less than 1 % ; ( ii ) pregnant women with advanced HIV infection require therapy ; ( iii ) combination therapy with at least 3 compounds significantly reduces morbidity and mortality compared with dual or monotherapy ; and ( iv ) the benefits of therapy for both the mother and the infant outweigh the risk .
	manualset3
240252	8	423574	15	NULL	NULL	NULL	NULL	less than 1 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Antiretroviral monotherapy and combination therapy is widely prescribed in pregnancy because : ( i ) with appropriate management , which includes antiretroviral therapy , the risk of mother-to-child transmission can be reduced from 15 to 25 % to less than 1 % ; ( ii ) pregnant women with advanced HIV infection require therapy ; ( iii ) combination therapy with at least 3 compounds significantly reduces morbidity and mortality compared with dual or monotherapy ; and ( iv ) the benefits of therapy for both the mother and the infant outweigh the risk .
	manualset3
240253	9	423574	15	NULL	NULL	0	NULL	pregnant women 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Antiretroviral monotherapy and combination therapy is widely prescribed in pregnancy because : ( i ) with appropriate management , which includes antiretroviral therapy , the risk of mother-to-child transmission can be reduced from 15 to 25 % to less than 1 % ; ( ii ) pregnant women with advanced HIV infection require therapy ; ( iii ) combination therapy with at least 3 compounds significantly reduces morbidity and mortality compared with dual or monotherapy ; and ( iv ) the benefits of therapy for both the mother and the infant outweigh the risk .
	manualset3
240254	10	423574	15	NULL	NULL	0	NULL	advanced HIV infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antiretroviral monotherapy and combination therapy is widely prescribed in pregnancy because : ( i ) with appropriate management , which includes antiretroviral therapy , the risk of mother-to-child transmission can be reduced from 15 to 25 % to less than 1 % ; ( ii ) pregnant women with advanced HIV infection require therapy ; ( iii ) combination therapy with at least 3 compounds significantly reduces morbidity and mortality compared with dual or monotherapy ; and ( iv ) the benefits of therapy for both the mother and the infant outweigh the risk .
	manualset3
240255	11	423574	15	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Antiretroviral monotherapy and combination therapy is widely prescribed in pregnancy because : ( i ) with appropriate management , which includes antiretroviral therapy , the risk of mother-to-child transmission can be reduced from 15 to 25 % to less than 1 % ; ( ii ) pregnant women with advanced HIV infection require therapy ; ( iii ) combination therapy with at least 3 compounds significantly reduces morbidity and mortality compared with dual or monotherapy ; and ( iv ) the benefits of therapy for both the mother and the infant outweigh the risk .
	manualset3
240256	12	423574	15	NULL	NULL	0	NULL	combination therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Antiretroviral monotherapy and combination therapy is widely prescribed in pregnancy because : ( i ) with appropriate management , which includes antiretroviral therapy , the risk of mother-to-child transmission can be reduced from 15 to 25 % to less than 1 % ; ( ii ) pregnant women with advanced HIV infection require therapy ; ( iii ) combination therapy with at least 3 compounds significantly reduces morbidity and mortality compared with dual or monotherapy ; and ( iv ) the benefits of therapy for both the mother and the infant outweigh the risk .
	manualset3
240257	13	423574	15	NULL	NULL	0	NULL	3 compounds	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Antiretroviral monotherapy and combination therapy is widely prescribed in pregnancy because : ( i ) with appropriate management , which includes antiretroviral therapy , the risk of mother-to-child transmission can be reduced from 15 to 25 % to less than 1 % ; ( ii ) pregnant women with advanced HIV infection require therapy ; ( iii ) combination therapy with at least 3 compounds significantly reduces morbidity and mortality compared with dual or monotherapy ; and ( iv ) the benefits of therapy for both the mother and the infant outweigh the risk .
	manualset3
240258	14	423574	15	NULL	NULL	0	NULL	 morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antiretroviral monotherapy and combination therapy is widely prescribed in pregnancy because : ( i ) with appropriate management , which includes antiretroviral therapy , the risk of mother-to-child transmission can be reduced from 15 to 25 % to less than 1 % ; ( ii ) pregnant women with advanced HIV infection require therapy ; ( iii ) combination therapy with at least 3 compounds significantly reduces morbidity and mortality compared with dual or monotherapy ; and ( iv ) the benefits of therapy for both the mother and the infant outweigh the risk .
	manualset3
240259	15	423574	15	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antiretroviral monotherapy and combination therapy is widely prescribed in pregnancy because : ( i ) with appropriate management , which includes antiretroviral therapy , the risk of mother-to-child transmission can be reduced from 15 to 25 % to less than 1 % ; ( ii ) pregnant women with advanced HIV infection require therapy ; ( iii ) combination therapy with at least 3 compounds significantly reduces morbidity and mortality compared with dual or monotherapy ; and ( iv ) the benefits of therapy for both the mother and the infant outweigh the risk .
	manualset3
240260	16	423574	15	NULL	NULL	0	NULL	dualtherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Antiretroviral monotherapy and combination therapy is widely prescribed in pregnancy because : ( i ) with appropriate management , which includes antiretroviral therapy , the risk of mother-to-child transmission can be reduced from 15 to 25 % to less than 1 % ; ( ii ) pregnant women with advanced HIV infection require therapy ; ( iii ) combination therapy with at least 3 compounds significantly reduces morbidity and mortality compared with dual or monotherapy ; and ( iv ) the benefits of therapy for both the mother and the infant outweigh the risk .
	manualset3
240261	17	423574	15	NULL	NULL	0	NULL	monotherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Antiretroviral monotherapy and combination therapy is widely prescribed in pregnancy because : ( i ) with appropriate management , which includes antiretroviral therapy , the risk of mother-to-child transmission can be reduced from 15 to 25 % to less than 1 % ; ( ii ) pregnant women with advanced HIV infection require therapy ; ( iii ) combination therapy with at least 3 compounds significantly reduces morbidity and mortality compared with dual or monotherapy ; and ( iv ) the benefits of therapy for both the mother and the infant outweigh the risk .
	manualset3
240262	18	423574	15	NULL	NULL	0	NULL	benefits of therapy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antiretroviral monotherapy and combination therapy is widely prescribed in pregnancy because : ( i ) with appropriate management , which includes antiretroviral therapy , the risk of mother-to-child transmission can be reduced from 15 to 25 % to less than 1 % ; ( ii ) pregnant women with advanced HIV infection require therapy ; ( iii ) combination therapy with at least 3 compounds significantly reduces morbidity and mortality compared with dual or monotherapy ; and ( iv ) the benefits of therapy for both the mother and the infant outweigh the risk .
	manualset3
240263	19	423574	15	NULL	NULL	0	NULL	mother 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Antiretroviral monotherapy and combination therapy is widely prescribed in pregnancy because : ( i ) with appropriate management , which includes antiretroviral therapy , the risk of mother-to-child transmission can be reduced from 15 to 25 % to less than 1 % ; ( ii ) pregnant women with advanced HIV infection require therapy ; ( iii ) combination therapy with at least 3 compounds significantly reduces morbidity and mortality compared with dual or monotherapy ; and ( iv ) the benefits of therapy for both the mother and the infant outweigh the risk .
	manualset3
240264	20	423574	15	NULL	NULL	0	NULL	infant	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Antiretroviral monotherapy and combination therapy is widely prescribed in pregnancy because : ( i ) with appropriate management , which includes antiretroviral therapy , the risk of mother-to-child transmission can be reduced from 15 to 25 % to less than 1 % ; ( ii ) pregnant women with advanced HIV infection require therapy ; ( iii ) combination therapy with at least 3 compounds significantly reduces morbidity and mortality compared with dual or monotherapy ; and ( iv ) the benefits of therapy for both the mother and the infant outweigh the risk .
	manualset3
240265	21	423574	15	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antiretroviral monotherapy and combination therapy is widely prescribed in pregnancy because : ( i ) with appropriate management , which includes antiretroviral therapy , the risk of mother-to-child transmission can be reduced from 15 to 25 % to less than 1 % ; ( ii ) pregnant women with advanced HIV infection require therapy ; ( iii ) combination therapy with at least 3 compounds significantly reduces morbidity and mortality compared with dual or monotherapy ; and ( iv ) the benefits of therapy for both the mother and the infant outweigh the risk .
	manualset3
240266	1	423575	15	NULL	NULL	0	NULL	Antisense IL-10	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Antisense IL-10 abrogates the inhibitory effects of IL-10 production by transfected tumor cells .
	manualset3
240267	2	423575	15	NULL	NULL	0	NULL	inhibitory effects of IL-10 production 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antisense IL-10 abrogates the inhibitory effects of IL-10 production by transfected tumor cells .
	manualset3
240268	3	423575	15	NULL	NULL	0	NULL	transfected tumor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Antisense IL-10 abrogates the inhibitory effects of IL-10 production by transfected tumor cells .
	manualset3
240280	1	423576	15	NULL	NULL	0	NULL	Antistaphylococcal activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antistaphylococcal activity of vancomycin and teicoplanin under anaerobic conditions .
	manualset3
240281	2	423576	15	NULL	NULL	0	NULL	vancomycin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Antistaphylococcal activity of vancomycin and teicoplanin under anaerobic conditions .
	manualset3
240282	3	423576	15	NULL	NULL	0	NULL	teicoplanin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Antistaphylococcal activity of vancomycin and teicoplanin under anaerobic conditions .
	manualset3
240283	4	423576	15	NULL	NULL	0	NULL	anaerobic conditions	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Antistaphylococcal activity of vancomycin and teicoplanin under anaerobic conditions .
	manualset3
240286	1	423577	15	NULL	NULL	NULL	NULL	Antitumor activity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Antitumor activity and long-term fate of chimeric antigen receptor-positive T cells in patients with neuroblastoma .
	manualset3
240290	2	423577	15	NULL	NULL	0	NULL	long-term fate 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antitumor activity and long-term fate of chimeric antigen receptor-positive T cells in patients with neuroblastoma .
	manualset3
240292	3	423577	15	NULL	NULL	0	NULL	chimeric antigen receptor-positive T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Antitumor activity and long-term fate of chimeric antigen receptor-positive T cells in patients with neuroblastoma .
	manualset3
240295	4	423577	15	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Antitumor activity and long-term fate of chimeric antigen receptor-positive T cells in patients with neuroblastoma .
	manualset3
240297	5	423577	15	NULL	NULL	0	NULL	neuroblastoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Antitumor activity and long-term fate of chimeric antigen receptor-positive T cells in patients with neuroblastoma .
	manualset3
240299	1	423578	15	NULL	NULL	0	NULL	Echo-tracking technology 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Echo-tracking technology for evaluating the impact of blood pressure on vascular endothelial function ) .
	manualset3
240303	3	423578	15	NULL	NULL	NULL	NULL	impact of blood pressure	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Echo-tracking technology for evaluating the impact of blood pressure on vascular endothelial function ) .
	manualset3
240305	4	423578	15	NULL	NULL	NULL	NULL	vascular endothelial function 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Echo-tracking technology for evaluating the impact of blood pressure on vascular endothelial function ) .
	manualset3
260695	2	423578	15	NULL	NULL	NULL	NULL	evaluating	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Echo-tracking technology for evaluating the impact of blood pressure on vascular endothelial function ) .
	manualset3
240323	1	423579	15	NULL	NULL	0	NULL	Antitumor pyrido ( 3 , 2-d ) ( 1 ) benzazepines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Antitumor pyrido ( 3 , 2-d ) ( 1 ) benzazepines : synthesis and in vitro activity of thiophene analogs .
	manualset3
240325	2	423579	15	NULL	NULL	0	NULL	synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antitumor pyrido ( 3 , 2-d ) ( 1 ) benzazepines : synthesis and in vitro activity of thiophene analogs .
	manualset3
240327	3	423579	15	NULL	NULL	0	NULL	in vitro activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antitumor pyrido ( 3 , 2-d ) ( 1 ) benzazepines : synthesis and in vitro activity of thiophene analogs .
	manualset3
240328	4	423579	15	NULL	NULL	0	NULL	thiophene analogs	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Antitumor pyrido ( 3 , 2-d ) ( 1 ) benzazepines : synthesis and in vitro activity of thiophene analogs .
	manualset3
240329	1	423580	15	NULL	NULL	0	NULL	Antiviral activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Antiviral activity of shiga toxin requires enzymatic activity and is associated with increased permeability of the target cells .
	manualset3
240332	2	423580	15	NULL	NULL	0	NULL	shiga toxin 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Antiviral activity of shiga toxin requires enzymatic activity and is associated with increased permeability of the target cells .
	manualset3
240333	3	423580	15	NULL	NULL	0	NULL	enzymatic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antiviral activity of shiga toxin requires enzymatic activity and is associated with increased permeability of the target cells .
	manualset3
240409	4	423580	15	NULL	NULL	0	NULL	permeability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Antiviral activity of shiga toxin requires enzymatic activity and is associated with increased permeability of the target cells .
	manualset3
240410	5	423580	15	NULL	NULL	0	NULL	target cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Antiviral activity of shiga toxin requires enzymatic activity and is associated with increased permeability of the target cells .
	manualset3
240412	1	423581	15	NULL	NULL	0	NULL	Anxiety	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Anxiety , depression , mood , personality , and generic health-related quality of life will also be assessed at baseline to provide preliminary evidence of validity .
	manualset3
240414	2	423581	15	NULL	NULL	0	NULL	depression	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Anxiety , depression , mood , personality , and generic health-related quality of life will also be assessed at baseline to provide preliminary evidence of validity .
	manualset3
240416	3	423581	15	NULL	NULL	0	NULL	mood	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Anxiety , depression , mood , personality , and generic health-related quality of life will also be assessed at baseline to provide preliminary evidence of validity .
	manualset3
240417	4	423581	15	NULL	NULL	0	NULL	personality	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Anxiety , depression , mood , personality , and generic health-related quality of life will also be assessed at baseline to provide preliminary evidence of validity .
	manualset3
240420	5	423581	15	NULL	NULL	0	NULL	generic health-related quality of life	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Anxiety , depression , mood , personality , and generic health-related quality of life will also be assessed at baseline to provide preliminary evidence of validity .
	manualset3
240423	6	423581	15	NULL	NULL	NULL	NULL	baseline	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Anxiety , depression , mood , personality , and generic health-related quality of life will also be assessed at baseline to provide preliminary evidence of validity .
	manualset3
240426	7	423581	15	NULL	NULL	0	NULL	preliminary evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Anxiety , depression , mood , personality , and generic health-related quality of life will also be assessed at baseline to provide preliminary evidence of validity .
	manualset3
240433	8	423581	15	NULL	NULL	0	NULL	validity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Anxiety , depression , mood , personality , and generic health-related quality of life will also be assessed at baseline to provide preliminary evidence of validity .
	manualset3
240438	2	423582	15	NULL	NULL	NULL	NULL	AS RNA	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Anyone considering the use of AS RNA , generated endogenously , to inhibit gene expression should plan to generate several independent transfectants with nonoverlapping sequences ; strategies that maximize both the transcription rate and the stability of the AS RNA are obviously desirable .
	manualset3
240440	3	423582	15	NULL	NULL	NULL	NULL	gene expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Anyone considering the use of AS RNA , generated endogenously , to inhibit gene expression should plan to generate several independent transfectants with nonoverlapping sequences ; strategies that maximize both the transcription rate and the stability of the AS RNA are obviously desirable .
	manualset3
240442	4	423582	15	NULL	NULL	NULL	NULL	independent transfectants	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Anyone considering the use of AS RNA , generated endogenously , to inhibit gene expression should plan to generate several independent transfectants with nonoverlapping sequences ; strategies that maximize both the transcription rate and the stability of the AS RNA are obviously desirable .
	manualset3
240443	5	423582	15	NULL	NULL	NULL	NULL	nonoverlapping sequences	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Anyone considering the use of AS RNA , generated endogenously , to inhibit gene expression should plan to generate several independent transfectants with nonoverlapping sequences ; strategies that maximize both the transcription rate and the stability of the AS RNA are obviously desirable .
	manualset3
240444	6	423582	15	NULL	NULL	NULL	NULL	strategies	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Anyone considering the use of AS RNA , generated endogenously , to inhibit gene expression should plan to generate several independent transfectants with nonoverlapping sequences ; strategies that maximize both the transcription rate and the stability of the AS RNA are obviously desirable .
	manualset3
240445	7	423582	15	NULL	NULL	NULL	NULL	transcription rate	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Anyone considering the use of AS RNA , generated endogenously , to inhibit gene expression should plan to generate several independent transfectants with nonoverlapping sequences ; strategies that maximize both the transcription rate and the stability of the AS RNA are obviously desirable .
	manualset3
240446	8	423582	15	NULL	NULL	NULL	NULL	stability	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Anyone considering the use of AS RNA , generated endogenously , to inhibit gene expression should plan to generate several independent transfectants with nonoverlapping sequences ; strategies that maximize both the transcription rate and the stability of the AS RNA are obviously desirable .
	manualset3
240448	9	423582	15	NULL	NULL	NULL	NULL	AS RNA 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Anyone considering the use of AS RNA , generated endogenously , to inhibit gene expression should plan to generate several independent transfectants with nonoverlapping sequences ; strategies that maximize both the transcription rate and the stability of the AS RNA are obviously desirable .
	manualset3
258527	1	423582	15	NULL	NULL	NULL	NULL	use 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Anyone considering the use of AS RNA , generated endogenously , to inhibit gene expression should plan to generate several independent transfectants with nonoverlapping sequences ; strategies that maximize both the transcription rate and the stability of the AS RNA are obviously desirable .
	manualset3
240449	1	423583	15	NULL	NULL	0	NULL	Aortic cGMP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Aortic cGMP was lowered in rats treated with L-NAME ( 530 + / - 120 fmol/mg protein , n = 12 , P & lt ; .05 ) and L-NAME plus quinapril ( 461 + / - 140 fmol/mg protein , n = 12 , P & lt ; .05 ) compared with controls ( 1798 + / - 522 fmol/mg protein , n = 12 ) .
	manualset3
240450	2	423583	15	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Aortic cGMP was lowered in rats treated with L-NAME ( 530 + / - 120 fmol/mg protein , n = 12 , P & lt ; .05 ) and L-NAME plus quinapril ( 461 + / - 140 fmol/mg protein , n = 12 , P & lt ; .05 ) compared with controls ( 1798 + / - 522 fmol/mg protein , n = 12 ) .
	manualset3
240451	3	423583	15	NULL	NULL	0	NULL	L-NAME	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Aortic cGMP was lowered in rats treated with L-NAME ( 530 + / - 120 fmol/mg protein , n = 12 , P & lt ; .05 ) and L-NAME plus quinapril ( 461 + / - 140 fmol/mg protein , n = 12 , P & lt ; .05 ) compared with controls ( 1798 + / - 522 fmol/mg protein , n = 12 ) .
	manualset3
240452	4	423583	15	NULL	NULL	NULL	NULL	530 + / - 120 fmol/mg protein	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Aortic cGMP was lowered in rats treated with L-NAME ( 530 + / - 120 fmol/mg protein , n = 12 , P & lt ; .05 ) and L-NAME plus quinapril ( 461 + / - 140 fmol/mg protein , n = 12 , P & lt ; .05 ) compared with controls ( 1798 + / - 522 fmol/mg protein , n = 12 ) .
	manualset3
240453	5	423583	15	NULL	NULL	0	NULL	n = 12	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Aortic cGMP was lowered in rats treated with L-NAME ( 530 + / - 120 fmol/mg protein , n = 12 , P & lt ; .05 ) and L-NAME plus quinapril ( 461 + / - 140 fmol/mg protein , n = 12 , P & lt ; .05 ) compared with controls ( 1798 + / - 522 fmol/mg protein , n = 12 ) .
	manualset3
240454	6	423583	15	NULL	NULL	0	NULL	P & lt ; .05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Aortic cGMP was lowered in rats treated with L-NAME ( 530 + / - 120 fmol/mg protein , n = 12 , P & lt ; .05 ) and L-NAME plus quinapril ( 461 + / - 140 fmol/mg protein , n = 12 , P & lt ; .05 ) compared with controls ( 1798 + / - 522 fmol/mg protein , n = 12 ) .
	manualset3
240455	7	423583	15	NULL	NULL	0	NULL	L-NAME	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Aortic cGMP was lowered in rats treated with L-NAME ( 530 + / - 120 fmol/mg protein , n = 12 , P & lt ; .05 ) and L-NAME plus quinapril ( 461 + / - 140 fmol/mg protein , n = 12 , P & lt ; .05 ) compared with controls ( 1798 + / - 522 fmol/mg protein , n = 12 ) .
	manualset3
240456	8	423583	15	NULL	NULL	0	NULL	quinapril	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Aortic cGMP was lowered in rats treated with L-NAME ( 530 + / - 120 fmol/mg protein , n = 12 , P & lt ; .05 ) and L-NAME plus quinapril ( 461 + / - 140 fmol/mg protein , n = 12 , P & lt ; .05 ) compared with controls ( 1798 + / - 522 fmol/mg protein , n = 12 ) .
	manualset3
240457	9	423583	15	NULL	NULL	0	NULL	461 + / - 140 fmol/mg protein	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Aortic cGMP was lowered in rats treated with L-NAME ( 530 + / - 120 fmol/mg protein , n = 12 , P & lt ; .05 ) and L-NAME plus quinapril ( 461 + / - 140 fmol/mg protein , n = 12 , P & lt ; .05 ) compared with controls ( 1798 + / - 522 fmol/mg protein , n = 12 ) .
	manualset3
240458	10	423583	15	NULL	NULL	0	NULL	n = 12	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Aortic cGMP was lowered in rats treated with L-NAME ( 530 + / - 120 fmol/mg protein , n = 12 , P & lt ; .05 ) and L-NAME plus quinapril ( 461 + / - 140 fmol/mg protein , n = 12 , P & lt ; .05 ) compared with controls ( 1798 + / - 522 fmol/mg protein , n = 12 ) .
	manualset3
240459	11	423583	15	NULL	NULL	0	NULL	P & lt ; .05 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Aortic cGMP was lowered in rats treated with L-NAME ( 530 + / - 120 fmol/mg protein , n = 12 , P & lt ; .05 ) and L-NAME plus quinapril ( 461 + / - 140 fmol/mg protein , n = 12 , P & lt ; .05 ) compared with controls ( 1798 + / - 522 fmol/mg protein , n = 12 ) .
	manualset3
240460	12	423583	15	NULL	NULL	0	NULL	controls	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Aortic cGMP was lowered in rats treated with L-NAME ( 530 + / - 120 fmol/mg protein , n = 12 , P & lt ; .05 ) and L-NAME plus quinapril ( 461 + / - 140 fmol/mg protein , n = 12 , P & lt ; .05 ) compared with controls ( 1798 + / - 522 fmol/mg protein , n = 12 ) .
	manualset3
240461	13	423583	15	NULL	NULL	0	NULL	1798 + / - 522 fmol/mg protein	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Aortic cGMP was lowered in rats treated with L-NAME ( 530 + / - 120 fmol/mg protein , n = 12 , P & lt ; .05 ) and L-NAME plus quinapril ( 461 + / - 140 fmol/mg protein , n = 12 , P & lt ; .05 ) compared with controls ( 1798 + / - 522 fmol/mg protein , n = 12 ) .
	manualset3
240462	14	423583	15	NULL	NULL	0	NULL	n = 12	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Aortic cGMP was lowered in rats treated with L-NAME ( 530 + / - 120 fmol/mg protein , n = 12 , P & lt ; .05 ) and L-NAME plus quinapril ( 461 + / - 140 fmol/mg protein , n = 12 , P & lt ; .05 ) compared with controls ( 1798 + / - 522 fmol/mg protein , n = 12 ) .
	manualset3
240463	1	423584	15	NULL	NULL	0	NULL	Aortic intramural hematoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Aortic intramural hematoma : from observation to therapeutic strategies .
	manualset3
240464	2	423584	15	NULL	NULL	0	NULL	observation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Aortic intramural hematoma : from observation to therapeutic strategies .
	manualset3
240465	3	423584	15	NULL	NULL	0	NULL	 therapeutic strategies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Aortic intramural hematoma : from observation to therapeutic strategies .
	manualset3
240466	1	423585	15	NULL	NULL	0	NULL	Aortic valve cyclic stretch	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Aortic valve cyclic stretch causes increased remodeling activity and enhanced serotonin receptor responsiveness .
	manualset3
240467	2	423585	15	NULL	NULL	0	NULL	remodeling activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Aortic valve cyclic stretch causes increased remodeling activity and enhanced serotonin receptor responsiveness .
	manualset3
240468	3	423585	15	NULL	NULL	0	NULL	serotonin receptor responsiveness	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Aortic valve cyclic stretch causes increased remodeling activity and enhanced serotonin receptor responsiveness .
	manualset3
240469	1	423586	15	NULL	NULL	0	NULL	Ed-Glu-Gate solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Ed-Glu-Gate solution for the taking of blood to be used in extracorporeal circulation ) .
	manualset3
240470	2	423586	15	NULL	NULL	NULL	NULL	taking of blood	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Ed-Glu-Gate solution for the taking of blood to be used in extracorporeal circulation ) .
	manualset3
240471	3	423586	15	NULL	NULL	NULL	NULL	extracorporeal circulation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Ed-Glu-Gate solution for the taking of blood to be used in extracorporeal circulation ) .
	manualset3
240472	1	423587	15	NULL	NULL	0	NULL	Aortic valve replacement	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Aortic valve replacement combined with the endoventricular patch technique for aortic valve stenosis complicated by ischemic heart disease .
	manualset3
240473	2	423587	15	NULL	NULL	0	NULL	endoventricular patch technique	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Aortic valve replacement combined with the endoventricular patch technique for aortic valve stenosis complicated by ischemic heart disease .
	manualset3
240474	3	423587	15	NULL	NULL	NULL	NULL	aortic valve stenosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Aortic valve replacement combined with the endoventricular patch technique for aortic valve stenosis complicated by ischemic heart disease .
	manualset3
240475	4	423587	15	NULL	NULL	0	NULL	ischemic heart disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Aortic valve replacement combined with the endoventricular patch technique for aortic valve stenosis complicated by ischemic heart disease .
	manualset3
240476	1	423588	15	NULL	NULL	NULL	NULL	Aortobipopliteal bypass	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Aortobipopliteal bypass via the obturator foramina .
	manualset3
240477	2	423588	15	NULL	NULL	NULL	NULL	obturator foramina	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Aortobipopliteal bypass via the obturator foramina .
	manualset3
240478	1	423589	15	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from its role in regulating SAR in the nucleus , a novel cytosolic function of NPR1 in cross-communication between SA - and JA-dependent defense signaling pathways has been identified .
	manualset3
240479	2	423589	15	NULL	NULL	0	NULL	regulating SAR 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from its role in regulating SAR in the nucleus , a novel cytosolic function of NPR1 in cross-communication between SA - and JA-dependent defense signaling pathways has been identified .
	manualset3
240480	3	423589	15	NULL	NULL	0	NULL	nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from its role in regulating SAR in the nucleus , a novel cytosolic function of NPR1 in cross-communication between SA - and JA-dependent defense signaling pathways has been identified .
	manualset3
240481	4	423589	15	NULL	NULL	0	NULL	function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from its role in regulating SAR in the nucleus , a novel cytosolic function of NPR1 in cross-communication between SA - and JA-dependent defense signaling pathways has been identified .
	manualset3
240482	5	423589	15	NULL	NULL	0	NULL	NPR1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from its role in regulating SAR in the nucleus , a novel cytosolic function of NPR1 in cross-communication between SA - and JA-dependent defense signaling pathways has been identified .
	manualset3
240483	6	423589	15	NULL	NULL	0	NULL	cross-communication	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from its role in regulating SAR in the nucleus , a novel cytosolic function of NPR1 in cross-communication between SA - and JA-dependent defense signaling pathways has been identified .
	manualset3
240484	7	423589	15	NULL	NULL	0	NULL	SA - and JA-dependent defense signaling pathways 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from its role in regulating SAR in the nucleus , a novel cytosolic function of NPR1 in cross-communication between SA - and JA-dependent defense signaling pathways has been identified .
	manualset3
240485	1	423590	15	NULL	NULL	0	NULL	energy homeostasis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from energy homeostasis leptin has been shown to be involved in a number of neuronal networks .
	manualset3
240486	2	423590	15	NULL	NULL	0	NULL	leptin	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from energy homeostasis leptin has been shown to be involved in a number of neuronal networks .
	manualset3
240487	3	423590	15	NULL	NULL	0	NULL	neuronal networks	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from energy homeostasis leptin has been shown to be involved in a number of neuronal networks .
	manualset3
240488	1	423591	15	NULL	NULL	0	NULL	etiochloroplast-specific accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from etiochloroplast-specific accumulation of the DPOR subunits , we described , in some detail , additional specific features of chlorophyll biosynthesis in the spruce seedlings that differ from those known in angiosperms .
	manualset3
240489	2	423591	15	NULL	NULL	0	NULL	DPOR subunits	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from etiochloroplast-specific accumulation of the DPOR subunits , we described , in some detail , additional specific features of chlorophyll biosynthesis in the spruce seedlings that differ from those known in angiosperms .
	manualset3
240490	3	423591	15	NULL	NULL	0	NULL	detail	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from etiochloroplast-specific accumulation of the DPOR subunits , we described , in some detail , additional specific features of chlorophyll biosynthesis in the spruce seedlings that differ from those known in angiosperms .
	manualset3
240491	4	423591	15	NULL	NULL	0	NULL	additional specific features	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from etiochloroplast-specific accumulation of the DPOR subunits , we described , in some detail , additional specific features of chlorophyll biosynthesis in the spruce seedlings that differ from those known in angiosperms .
	manualset3
240492	5	423591	15	NULL	NULL	0	NULL	chlorophyll biosynthesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from etiochloroplast-specific accumulation of the DPOR subunits , we described , in some detail , additional specific features of chlorophyll biosynthesis in the spruce seedlings that differ from those known in angiosperms .
	manualset3
240493	6	423591	15	NULL	NULL	0	NULL	spruce seedlings	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from etiochloroplast-specific accumulation of the DPOR subunits , we described , in some detail , additional specific features of chlorophyll biosynthesis in the spruce seedlings that differ from those known in angiosperms .
	manualset3
240494	7	423591	15	NULL	NULL	0	NULL	angiosperms 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from etiochloroplast-specific accumulation of the DPOR subunits , we described , in some detail , additional specific features of chlorophyll biosynthesis in the spruce seedlings that differ from those known in angiosperms .
	manualset3
240495	1	423592	15	NULL	NULL	0	NULL	control material	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from the control material , the experimental resin-modified glass-ionomer material , V-66 , had the highest radiopacity of all the materials tested .
	manualset3
240496	2	423592	15	NULL	NULL	0	NULL	experimental resin-modified glass-ionomer material	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from the control material , the experimental resin-modified glass-ionomer material , V-66 , had the highest radiopacity of all the materials tested .
	manualset3
240497	3	423592	15	NULL	NULL	0	NULL	V-66	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from the control material , the experimental resin-modified glass-ionomer material , V-66 , had the highest radiopacity of all the materials tested .
	manualset3
240498	4	423592	15	NULL	NULL	0	NULL	radiopacity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from the control material , the experimental resin-modified glass-ionomer material , V-66 , had the highest radiopacity of all the materials tested .
	manualset3
240499	5	423592	15	NULL	NULL	0	NULL	materials	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from the control material , the experimental resin-modified glass-ionomer material , V-66 , had the highest radiopacity of all the materials tested .
	manualset3
240500	1	423593	15	NULL	NULL	0	NULL	samples	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from this , in samples with a longer storage interval and especially in postmortem specimens , higher levels can be measured due to GHB generation during this postmortem interval or storage time .
	manualset3
240501	2	423593	15	NULL	NULL	0	NULL	storage interval	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from this , in samples with a longer storage interval and especially in postmortem specimens , higher levels can be measured due to GHB generation during this postmortem interval or storage time .
	manualset3
240502	3	423593	15	NULL	NULL	0	NULL	postmortem specimens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from this , in samples with a longer storage interval and especially in postmortem specimens , higher levels can be measured due to GHB generation during this postmortem interval or storage time .
	manualset3
240503	4	423593	15	NULL	NULL	0	NULL	levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from this , in samples with a longer storage interval and especially in postmortem specimens , higher levels can be measured due to GHB generation during this postmortem interval or storage time .
	manualset3
240505	5	423593	15	NULL	NULL	0	NULL	GHB generation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from this , in samples with a longer storage interval and especially in postmortem specimens , higher levels can be measured due to GHB generation during this postmortem interval or storage time .
	manualset3
240506	6	423593	15	NULL	NULL	0	NULL	postmortem interval 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from this , in samples with a longer storage interval and especially in postmortem specimens , higher levels can be measured due to GHB generation during this postmortem interval or storage time .
	manualset3
240507	7	423593	15	NULL	NULL	0	NULL	storage time 	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Apart from this , in samples with a longer storage interval and especially in postmortem specimens , higher levels can be measured due to GHB generation during this postmortem interval or storage time .
	manualset3
240509	1	423594	15	NULL	NULL	NULL	NULL	Apheresis products	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Apheresis products contained 0.7 % + / - 0.2 % SD of myeloma cells ( range , 0.2 % to 2.7 % ) .
	manualset3
240512	2	423594	15	NULL	NULL	0	NULL	0.7 % + / - 0.2 % SD	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Apheresis products contained 0.7 % + / - 0.2 % SD of myeloma cells ( range , 0.2 % to 2.7 % ) .
	manualset3
240513	3	423594	15	NULL	NULL	0	NULL	myeloma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Apheresis products contained 0.7 % + / - 0.2 % SD of myeloma cells ( range , 0.2 % to 2.7 % ) .
	manualset3
240514	4	423594	15	NULL	NULL	0	NULL	range , 0.2 % to 2.7 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Apheresis products contained 0.7 % + / - 0.2 % SD of myeloma cells ( range , 0.2 % to 2.7 % ) .
	manualset3
240515	1	423595	15	NULL	NULL	0	NULL	Aphidophagous Syrphidae larvae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Aphidophagous Syrphidae larvae collected on leaves ofkale infested by L. pseudobrassicae belong to the species Allograpta exotica ( Wiedemann ) and Ocyptamus gastrostactus ( Wiedemann ) .
	manualset3
240516	2	423595	15	NULL	NULL	0	NULL	leaves ofkale	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Aphidophagous Syrphidae larvae collected on leaves ofkale infested by L. pseudobrassicae belong to the species Allograpta exotica ( Wiedemann ) and Ocyptamus gastrostactus ( Wiedemann ) .
	manualset3
240517	3	423595	15	NULL	NULL	0	NULL	L. pseudobrassicae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Aphidophagous Syrphidae larvae collected on leaves ofkale infested by L. pseudobrassicae belong to the species Allograpta exotica ( Wiedemann ) and Ocyptamus gastrostactus ( Wiedemann ) .
	manualset3
240518	4	423595	15	NULL	NULL	0	NULL	species Allograpta exotica	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Aphidophagous Syrphidae larvae collected on leaves ofkale infested by L. pseudobrassicae belong to the species Allograpta exotica ( Wiedemann ) and Ocyptamus gastrostactus ( Wiedemann ) .
	manualset3
240519	5	423595	15	NULL	NULL	0	NULL	Wiedemann	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Aphidophagous Syrphidae larvae collected on leaves ofkale infested by L. pseudobrassicae belong to the species Allograpta exotica ( Wiedemann ) and Ocyptamus gastrostactus ( Wiedemann ) .
	manualset3
240520	6	423595	15	NULL	NULL	0	NULL	Ocyptamus gastrostactus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Aphidophagous Syrphidae larvae collected on leaves ofkale infested by L. pseudobrassicae belong to the species Allograpta exotica ( Wiedemann ) and Ocyptamus gastrostactus ( Wiedemann ) .
	manualset3
240521	7	423595	15	NULL	NULL	0	NULL	Wiedemann	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Aphidophagous Syrphidae larvae collected on leaves ofkale infested by L. pseudobrassicae belong to the species Allograpta exotica ( Wiedemann ) and Ocyptamus gastrostactus ( Wiedemann ) .
	manualset3
240522	1	423596	15	NULL	NULL	NULL	NULL	Apical movements 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Apical and incisal vertical movements and increase in incisor proclination were the strong predictors of external apical root resorption for each regression model .
	manualset3
240523	2	423596	15	NULL	NULL	NULL	NULL	incisal vertical movements	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Apical and incisal vertical movements and increase in incisor proclination were the strong predictors of external apical root resorption for each regression model .
	manualset3
240524	3	423596	15	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Apical and incisal vertical movements and increase in incisor proclination were the strong predictors of external apical root resorption for each regression model .
	manualset3
240525	4	423596	15	NULL	NULL	0	NULL	incisor proclination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Apical and incisal vertical movements and increase in incisor proclination were the strong predictors of external apical root resorption for each regression model .
	manualset3
240526	5	423596	15	NULL	NULL	0	NULL	strong predictors of external apical root resorption	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Apical and incisal vertical movements and increase in incisor proclination were the strong predictors of external apical root resorption for each regression model .
	manualset3
240527	6	423596	15	NULL	NULL	NULL	NULL	regression model 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Apical and incisal vertical movements and increase in incisor proclination were the strong predictors of external apical root resorption for each regression model .
	manualset3
240528	1	423597	15	NULL	NULL	0	NULL	Education	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Education -- current demands of role as examiner ) .
	manualset3
240529	2	423597	15	NULL	NULL	0	NULL	demands	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Education -- current demands of role as examiner ) .
	manualset3
240530	3	423597	15	NULL	NULL	NULL	NULL	role	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Education -- current demands of role as examiner ) .
	manualset3
240596	4	423597	15	NULL	NULL	0	NULL	examiner	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( Education -- current demands of role as examiner ) .
	manualset3
240531	1	423598	15	NULL	NULL	0	NULL	ApoB	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	ApoB isolated by this procedure was essentially identical to apoB from autologous LDL with respect to molecular weight , secondary structure , amino acid composition , and sialic acid content .
	manualset3
240532	2	423598	15	NULL	NULL	0	NULL	procedure	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	ApoB isolated by this procedure was essentially identical to apoB from autologous LDL with respect to molecular weight , secondary structure , amino acid composition , and sialic acid content .
	manualset3
240533	3	423598	15	NULL	NULL	0	NULL	apoB	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	ApoB isolated by this procedure was essentially identical to apoB from autologous LDL with respect to molecular weight , secondary structure , amino acid composition , and sialic acid content .
	manualset3
240534	4	423598	15	NULL	NULL	0	NULL	autologous LDL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	ApoB isolated by this procedure was essentially identical to apoB from autologous LDL with respect to molecular weight , secondary structure , amino acid composition , and sialic acid content .
	manualset3
240535	5	423598	15	NULL	NULL	0	NULL	molecular weight	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	ApoB isolated by this procedure was essentially identical to apoB from autologous LDL with respect to molecular weight , secondary structure , amino acid composition , and sialic acid content .
	manualset3
240536	6	423598	15	NULL	NULL	NULL	NULL	secondary structure	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ApoB isolated by this procedure was essentially identical to apoB from autologous LDL with respect to molecular weight , secondary structure , amino acid composition , and sialic acid content .
	manualset3
240537	7	423598	15	NULL	NULL	0	NULL	amino acid composition 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	ApoB isolated by this procedure was essentially identical to apoB from autologous LDL with respect to molecular weight , secondary structure , amino acid composition , and sialic acid content .
	manualset3
240538	8	423598	15	NULL	NULL	0	NULL	sialic acid content	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	ApoB isolated by this procedure was essentially identical to apoB from autologous LDL with respect to molecular weight , secondary structure , amino acid composition , and sialic acid content .
	manualset3
240539	1	423599	15	NULL	NULL	0	NULL	Apocrine gland cyst 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Apocrine gland cyst with hemosiderotic dermatofibroma-like stroma : report of two cases .
	manualset3
240540	2	423599	15	NULL	NULL	NULL	NULL	hemosiderotic dermatofibroma-like stroma	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Apocrine gland cyst with hemosiderotic dermatofibroma-like stroma : report of two cases .
	manualset3
240541	3	423599	15	NULL	NULL	0	NULL	report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Apocrine gland cyst with hemosiderotic dermatofibroma-like stroma : report of two cases .
	manualset3
240542	4	423599	15	NULL	NULL	0	NULL	two cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Apocrine gland cyst with hemosiderotic dermatofibroma-like stroma : report of two cases .
	manualset3
240543	1	423600	15	NULL	NULL	0	NULL	Apolipoprotein C-II	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Apolipoprotein C-II , albumin and immunoglobulin G , which are also decisive plasma proteins with regard to site-specific drug delivery of intravenously injected carriers to the brain , are compared with regard to adsorption .
	manualset3
240544	2	423600	15	NULL	NULL	0	NULL	albumin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Apolipoprotein C-II , albumin and immunoglobulin G , which are also decisive plasma proteins with regard to site-specific drug delivery of intravenously injected carriers to the brain , are compared with regard to adsorption .
	manualset3
240545	3	423600	15	NULL	NULL	0	NULL	immunoglobulin G	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Apolipoprotein C-II , albumin and immunoglobulin G , which are also decisive plasma proteins with regard to site-specific drug delivery of intravenously injected carriers to the brain , are compared with regard to adsorption .
	manualset3
240546	4	423600	15	NULL	NULL	0	NULL	plasma proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Apolipoprotein C-II , albumin and immunoglobulin G , which are also decisive plasma proteins with regard to site-specific drug delivery of intravenously injected carriers to the brain , are compared with regard to adsorption .
	manualset3
240547	5	423600	15	NULL	NULL	0	NULL	site-specific drug delivery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Apolipoprotein C-II , albumin and immunoglobulin G , which are also decisive plasma proteins with regard to site-specific drug delivery of intravenously injected carriers to the brain , are compared with regard to adsorption .
	manualset3
240548	6	423600	15	NULL	NULL	0	NULL	intravenously injected carriers 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Apolipoprotein C-II , albumin and immunoglobulin G , which are also decisive plasma proteins with regard to site-specific drug delivery of intravenously injected carriers to the brain , are compared with regard to adsorption .
	manualset3
240549	7	423600	15	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Apolipoprotein C-II , albumin and immunoglobulin G , which are also decisive plasma proteins with regard to site-specific drug delivery of intravenously injected carriers to the brain , are compared with regard to adsorption .
	manualset3
240550	8	423600	15	NULL	NULL	0	NULL	adsorption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apolipoprotein C-II , albumin and immunoglobulin G , which are also decisive plasma proteins with regard to site-specific drug delivery of intravenously injected carriers to the brain , are compared with regard to adsorption .
	manualset3
240551	1	423601	15	NULL	NULL	0	NULL	Apolipoprotein E ( apoE )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Apolipoprotein E ( apoE ) down-regulates microglial activation and the secretion of inflammatory molecules in an isoform specific fashion ( E2 ) E3 ) E4 ) ; the E4 isoform is over-represented in Alzheimer cases while E2 is under-represented .
	manualset3
240552	2	423601	15	NULL	NULL	0	NULL	microglial activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apolipoprotein E ( apoE ) down-regulates microglial activation and the secretion of inflammatory molecules in an isoform specific fashion ( E2 ) E3 ) E4 ) ; the E4 isoform is over-represented in Alzheimer cases while E2 is under-represented .
	manualset3
240553	3	423601	15	NULL	NULL	0	NULL	secretion of inflammatory molecules	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apolipoprotein E ( apoE ) down-regulates microglial activation and the secretion of inflammatory molecules in an isoform specific fashion ( E2 ) E3 ) E4 ) ; the E4 isoform is over-represented in Alzheimer cases while E2 is under-represented .
	manualset3
240554	4	423601	15	NULL	NULL	0	NULL	isoform specific fashion ( E2 ) E3 ) E4 )	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apolipoprotein E ( apoE ) down-regulates microglial activation and the secretion of inflammatory molecules in an isoform specific fashion ( E2 ) E3 ) E4 ) ; the E4 isoform is over-represented in Alzheimer cases while E2 is under-represented .
	manualset3
240555	5	423601	15	NULL	NULL	0	NULL	E4 isoform	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Apolipoprotein E ( apoE ) down-regulates microglial activation and the secretion of inflammatory molecules in an isoform specific fashion ( E2 ) E3 ) E4 ) ; the E4 isoform is over-represented in Alzheimer cases while E2 is under-represented .
	manualset3
240556	6	423601	15	NULL	NULL	0	NULL	Alzheimer cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Apolipoprotein E ( apoE ) down-regulates microglial activation and the secretion of inflammatory molecules in an isoform specific fashion ( E2 ) E3 ) E4 ) ; the E4 isoform is over-represented in Alzheimer cases while E2 is under-represented .
	manualset3
240557	7	423601	15	NULL	NULL	0	NULL	E2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Apolipoprotein E ( apoE ) down-regulates microglial activation and the secretion of inflammatory molecules in an isoform specific fashion ( E2 ) E3 ) E4 ) ; the E4 isoform is over-represented in Alzheimer cases while E2 is under-represented .
	manualset3
240558	1	423602	15	NULL	NULL	0	NULL	Apolipoprotein E epsilon 4 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Apolipoprotein E epsilon 4 and fatal cerebral amyloid angiopathy associated with dementia pugilistica .
	manualset3
240559	2	423602	15	NULL	NULL	0	NULL	fatal cerebral amyloid angiopathy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Apolipoprotein E epsilon 4 and fatal cerebral amyloid angiopathy associated with dementia pugilistica .
	manualset3
240560	3	423602	15	NULL	NULL	0	NULL	dementia pugilistica	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Apolipoprotein E epsilon 4 and fatal cerebral amyloid angiopathy associated with dementia pugilistica .
	manualset3
240561	1	423603	15	NULL	NULL	0	NULL	Apolipoprotein O	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Apolipoprotein O promoted cholesterol efflux from macrophage cells .
	manualset3
240562	2	423603	15	NULL	NULL	0	NULL	cholesterol efflux	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apolipoprotein O promoted cholesterol efflux from macrophage cells .
	manualset3
240563	3	423603	15	NULL	NULL	0	NULL	macrophage cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Apolipoprotein O promoted cholesterol efflux from macrophage cells .
	manualset3
240564	1	423604	15	NULL	NULL	0	NULL	Educational reform 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Educational reform in medical education -- effects of the 8th revision of the medical approbation regulation on the psychosomatic/psychotherapy specialty ) .
	manualset3
240565	2	423604	15	NULL	NULL	0	NULL	medical education 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Educational reform in medical education -- effects of the 8th revision of the medical approbation regulation on the psychosomatic/psychotherapy specialty ) .
	manualset3
240566	3	423604	15	NULL	NULL	0	NULL	effects of the 8th revision	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Educational reform in medical education -- effects of the 8th revision of the medical approbation regulation on the psychosomatic/psychotherapy specialty ) .
	manualset3
240567	4	423604	15	NULL	NULL	NULL	NULL	medical approbation regulation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Educational reform in medical education -- effects of the 8th revision of the medical approbation regulation on the psychosomatic/psychotherapy specialty ) .
	manualset3
240568	5	423604	15	NULL	NULL	0	NULL	psychosomatic specialty	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Educational reform in medical education -- effects of the 8th revision of the medical approbation regulation on the psychosomatic/psychotherapy specialty ) .
	manualset3
240569	6	423604	15	NULL	NULL	0	NULL	psychotherapy specialty 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Educational reform in medical education -- effects of the 8th revision of the medical approbation regulation on the psychosomatic/psychotherapy specialty ) .
	manualset3
240570	1	423605	15	NULL	NULL	0	NULL	Apoptin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptin , a small protein derived from chicken anemia virus , can specifically induce apoptosis in transformed cells or tumor cells , but not in normal cells .
	manualset3
240571	2	423605	15	NULL	NULL	0	NULL	small protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptin , a small protein derived from chicken anemia virus , can specifically induce apoptosis in transformed cells or tumor cells , but not in normal cells .
	manualset3
240572	3	423605	15	NULL	NULL	0	NULL	chicken anemia virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptin , a small protein derived from chicken anemia virus , can specifically induce apoptosis in transformed cells or tumor cells , but not in normal cells .
	manualset3
240573	4	423605	15	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptin , a small protein derived from chicken anemia virus , can specifically induce apoptosis in transformed cells or tumor cells , but not in normal cells .
	manualset3
240574	5	423605	15	NULL	NULL	0	NULL	transformed cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptin , a small protein derived from chicken anemia virus , can specifically induce apoptosis in transformed cells or tumor cells , but not in normal cells .
	manualset3
240575	6	423605	15	NULL	NULL	0	NULL	tumor cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptin , a small protein derived from chicken anemia virus , can specifically induce apoptosis in transformed cells or tumor cells , but not in normal cells .
	manualset3
240576	7	423605	15	NULL	NULL	0	NULL	normal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptin , a small protein derived from chicken anemia virus , can specifically induce apoptosis in transformed cells or tumor cells , but not in normal cells .
	manualset3
240577	1	423606	15	NULL	NULL	0	NULL	Apoptosis-induced alkalinization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptosis-induced alkalinization by the Na + / H + exchanger isoform 1 is mediated through phosphorylation of amino acids Ser726 and Ser729 .
	manualset3
240578	2	423606	15	NULL	NULL	0	NULL	Na + / H + exchanger isoform 1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptosis-induced alkalinization by the Na + / H + exchanger isoform 1 is mediated through phosphorylation of amino acids Ser726 and Ser729 .
	manualset3
240579	3	423606	15	NULL	NULL	0	NULL	phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptosis-induced alkalinization by the Na + / H + exchanger isoform 1 is mediated through phosphorylation of amino acids Ser726 and Ser729 .
	manualset3
240580	4	423606	15	NULL	NULL	NULL	NULL	amino acids Ser726	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Apoptosis-induced alkalinization by the Na + / H + exchanger isoform 1 is mediated through phosphorylation of amino acids Ser726 and Ser729 .
	manualset3
240581	5	423606	15	NULL	NULL	0	NULL	amino acid Ser729	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptosis-induced alkalinization by the Na + / H + exchanger isoform 1 is mediated through phosphorylation of amino acids Ser726 and Ser729 .
	manualset3
240582	1	423607	15	NULL	NULL	0	NULL	Apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptosis in kidney and pancreas allograft biopsies .
	manualset3
240583	2	423607	15	NULL	NULL	0	NULL	kidney allograft biopsies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptosis in kidney and pancreas allograft biopsies .
	manualset3
240584	3	423607	15	NULL	NULL	0	NULL	pancreas allograft biopsies 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptosis in kidney and pancreas allograft biopsies .
	manualset3
240585	1	423608	15	NULL	NULL	0	NULL	Apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptosis is characterized by cell shrinkage , nuclear condensation , DNA-fragmentation and apoptotic body formation .
	manualset3
240586	2	423608	15	NULL	NULL	0	NULL	cell shrinkage 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptosis is characterized by cell shrinkage , nuclear condensation , DNA-fragmentation and apoptotic body formation .
	manualset3
240587	3	423608	15	NULL	NULL	0	NULL	nuclear condensation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptosis is characterized by cell shrinkage , nuclear condensation , DNA-fragmentation and apoptotic body formation .
	manualset3
240588	4	423608	15	NULL	NULL	0	NULL	DNA-fragmentation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptosis is characterized by cell shrinkage , nuclear condensation , DNA-fragmentation and apoptotic body formation .
	manualset3
240589	5	423608	15	NULL	NULL	0	NULL	apoptotic body formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptosis is characterized by cell shrinkage , nuclear condensation , DNA-fragmentation and apoptotic body formation .
	manualset3
240590	1	423609	15	NULL	NULL	0	NULL	Apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptosis is essential to eliminate secretory epithelial cells during the involution of the mammary gland .
	manualset3
240591	2	423609	15	NULL	NULL	0	NULL	secretory epithelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptosis is essential to eliminate secretory epithelial cells during the involution of the mammary gland .
	manualset3
240592	3	423609	15	NULL	NULL	0	NULL	involution of the mammary gland	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptosis is essential to eliminate secretory epithelial cells during the involution of the mammary gland .
	manualset3
240593	1	423610	15	NULL	NULL	0	NULL	Apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptosis occurred as early as 1h after PDT through activation of intrinsic pathways , followed by activation of extrinsic , caspase-12-dependent and caspase-independent pathways , and by autophagy .
	manualset3
240594	2	423610	15	NULL	NULL	0	NULL	1h after PDT 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptosis occurred as early as 1h after PDT through activation of intrinsic pathways , followed by activation of extrinsic , caspase-12-dependent and caspase-independent pathways , and by autophagy .
	manualset3
240595	3	423610	15	NULL	NULL	0	NULL	activation of intrinsic pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptosis occurred as early as 1h after PDT through activation of intrinsic pathways , followed by activation of extrinsic , caspase-12-dependent and caspase-independent pathways , and by autophagy .
	manualset3
240597	4	423610	15	NULL	NULL	0	NULL	activation of extrinsic pathways 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptosis occurred as early as 1h after PDT through activation of intrinsic pathways , followed by activation of extrinsic , caspase-12-dependent and caspase-independent pathways , and by autophagy .
	manualset3
240598	5	423610	15	NULL	NULL	0	NULL	caspase-12-dependent pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptosis occurred as early as 1h after PDT through activation of intrinsic pathways , followed by activation of extrinsic , caspase-12-dependent and caspase-independent pathways , and by autophagy .
	manualset3
240599	6	423610	15	NULL	NULL	0	NULL	caspase-independent pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptosis occurred as early as 1h after PDT through activation of intrinsic pathways , followed by activation of extrinsic , caspase-12-dependent and caspase-independent pathways , and by autophagy .
	manualset3
240600	7	423610	15	NULL	NULL	0	NULL	autophagy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptosis occurred as early as 1h after PDT through activation of intrinsic pathways , followed by activation of extrinsic , caspase-12-dependent and caspase-independent pathways , and by autophagy .
	manualset3
240601	1	423611	15	NULL	NULL	0	NULL	Apoptotic DNA fragmentation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptotic DNA fragmentation was detected by TUNEL staining .
	manualset3
240602	2	423611	15	NULL	NULL	0	NULL	TUNEL staining	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptotic DNA fragmentation was detected by TUNEL staining .
	manualset3
240603	1	423612	15	NULL	NULL	0	NULL	Effect of 1 , 3 butylene glycol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of 1 , 3 butylene glycol on reproduction in rats ) .
	manualset3
240604	2	423612	15	NULL	NULL	0	NULL	reproduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of 1 , 3 butylene glycol on reproduction in rats ) .
	manualset3
240605	3	423612	15	NULL	NULL	0	NULL	rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of 1 , 3 butylene glycol on reproduction in rats ) .
	manualset3
240606	1	423613	15	NULL	NULL	0	NULL	Apoptotic neuronal death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptotic neuronal death was induced by changing the medium to that containing 5.6 mM KCl without serum .
	manualset3
240607	2	423613	15	NULL	NULL	0	NULL	medium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptotic neuronal death was induced by changing the medium to that containing 5.6 mM KCl without serum .
	manualset3
240608	3	423613	15	NULL	NULL	0	NULL	5.6 mM KCl	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptotic neuronal death was induced by changing the medium to that containing 5.6 mM KCl without serum .
	manualset3
240610	4	423613	15	NULL	NULL	0	NULL	 serum 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Apoptotic neuronal death was induced by changing the medium to that containing 5.6 mM KCl without serum .
	manualset3
240613	1	423614	15	NULL	NULL	NULL	NULL	Apparent digestibilities 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Apparent digestibilities of dispensable amino acids were similar for SDE , PP , and SBM except proline and alanine .
	manualset3
240615	2	423614	15	NULL	NULL	0	NULL	dispensable amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Apparent digestibilities of dispensable amino acids were similar for SDE , PP , and SBM except proline and alanine .
	manualset3
240618	3	423614	15	NULL	NULL	0	NULL	SDE	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Apparent digestibilities of dispensable amino acids were similar for SDE , PP , and SBM except proline and alanine .
	manualset3
240619	4	423614	15	NULL	NULL	0	NULL	PP 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Apparent digestibilities of dispensable amino acids were similar for SDE , PP , and SBM except proline and alanine .
	manualset3
240621	5	423614	15	NULL	NULL	0	NULL	SBM	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Apparent digestibilities of dispensable amino acids were similar for SDE , PP , and SBM except proline and alanine .
	manualset3
240623	6	423614	15	NULL	NULL	0	NULL	proline	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Apparent digestibilities of dispensable amino acids were similar for SDE , PP , and SBM except proline and alanine .
	manualset3
240626	7	423614	15	NULL	NULL	0	NULL	alanine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Apparent digestibilities of dispensable amino acids were similar for SDE , PP , and SBM except proline and alanine .
	manualset3
240632	1	423615	15	NULL	NULL	0	NULL	HSV-2	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Apparently , HSV-2 is a rare inhabitant of periodontal sites .
	manualset3
240635	2	423615	15	NULL	NULL	0	NULL	inhabitant	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Apparently , HSV-2 is a rare inhabitant of periodontal sites .
	manualset3
240636	3	423615	15	NULL	NULL	0	NULL	periodontal sites 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Apparently , HSV-2 is a rare inhabitant of periodontal sites .
	manualset3
240643	1	423616	15	NULL	NULL	0	NULL	effect of training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Apparently , the effect of training was greater than calcium intake ( p & lt ; 0.05 ) .
	manualset3
240646	2	423616	15	NULL	NULL	NULL	NULL	calcium intake	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Apparently , the effect of training was greater than calcium intake ( p & lt ; 0.05 ) .
	manualset3
260700	3	423616	15	NULL	NULL	NULL	NULL	( p & lt ; 0.05 )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Apparently , the effect of training was greater than calcium intake ( p & lt ; 0.05 ) .
	manualset3
240650	1	423617	15	NULL	NULL	0	NULL	passive listening	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Apparently passive listening to lateralized natural sounds with a potential biological relevance led to an activation of motor networks involved in the automatic preparation for orientating .
	manualset3
240651	2	423617	15	NULL	NULL	0	NULL	lateralized natural sounds 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Apparently passive listening to lateralized natural sounds with a potential biological relevance led to an activation of motor networks involved in the automatic preparation for orientating .
	manualset3
240652	3	423617	15	NULL	NULL	0	NULL	biological relevance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apparently passive listening to lateralized natural sounds with a potential biological relevance led to an activation of motor networks involved in the automatic preparation for orientating .
	manualset3
240653	4	423617	15	NULL	NULL	NULL	NULL	activation of motor networks	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Apparently passive listening to lateralized natural sounds with a potential biological relevance led to an activation of motor networks involved in the automatic preparation for orientating .
	manualset3
240654	5	423617	15	NULL	NULL	0	NULL	automatic preparation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Apparently passive listening to lateralized natural sounds with a potential biological relevance led to an activation of motor networks involved in the automatic preparation for orientating .
	manualset3
260701	6	423617	15	NULL	NULL	NULL	NULL	orientating	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Apparently passive listening to lateralized natural sounds with a potential biological relevance led to an activation of motor networks involved in the automatic preparation for orientating .
	manualset3
240655	1	423618	15	NULL	NULL	0	NULL	Appearance 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Appearance of a ventricular 5-HT4 receptor-mediated inotropic response to serotonin in heart failure .
	manualset3
240656	2	423618	15	NULL	NULL	0	NULL	ventricular 5-HT4 receptor-mediated inotropic response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Appearance of a ventricular 5-HT4 receptor-mediated inotropic response to serotonin in heart failure .
	manualset3
240657	3	423618	15	NULL	NULL	NULL	NULL	serotonin	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Appearance of a ventricular 5-HT4 receptor-mediated inotropic response to serotonin in heart failure .
	manualset3
240658	4	423618	15	NULL	NULL	0	NULL	heart failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Appearance of a ventricular 5-HT4 receptor-mediated inotropic response to serotonin in heart failure .
	manualset3
240659	1	423619	15	NULL	NULL	NULL	NULL	Application of non-invasive examination 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Application and evaluation of non-invasive examination for Budd-Chiari syndrome .
	manualset3
240660	2	423619	15	NULL	NULL	0	NULL	evaluation of non-invasive examination	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Application and evaluation of non-invasive examination for Budd-Chiari syndrome .
	manualset3
240662	3	423619	15	NULL	NULL	0	NULL	Budd-Chiari syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Application and evaluation of non-invasive examination for Budd-Chiari syndrome .
	manualset3
240665	1	423620	15	NULL	NULL	0	NULL	Application of NiSO4 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of NiSO4 to the cytoplasmic face of inside-out membrane patches did not induce any currents .
	manualset3
240666	2	423620	15	NULL	NULL	NULL	NULL	cytoplasmic face of inside-out membrane patches	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Application of NiSO4 to the cytoplasmic face of inside-out membrane patches did not induce any currents .
	manualset3
240669	3	423620	15	NULL	NULL	0	NULL	currents	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of NiSO4 to the cytoplasmic face of inside-out membrane patches did not induce any currents .
	manualset3
240672	1	423621	15	NULL	NULL	0	NULL	Application of a microfluidic reaction system	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of a microfluidic reaction system for CdSe nanocrystal preparation : their growth kinetics and photoluminescence analysis .
	manualset3
240673	2	423621	15	NULL	NULL	0	NULL	CdSe nanocrystal preparation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of a microfluidic reaction system for CdSe nanocrystal preparation : their growth kinetics and photoluminescence analysis .
	manualset3
240674	3	423621	15	NULL	NULL	0	NULL	growth kinetics	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of a microfluidic reaction system for CdSe nanocrystal preparation : their growth kinetics and photoluminescence analysis .
	manualset3
240675	4	423621	15	NULL	NULL	0	NULL	photoluminescence analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of a microfluidic reaction system for CdSe nanocrystal preparation : their growth kinetics and photoluminescence analysis .
	manualset3
240676	1	423622	15	NULL	NULL	NULL	NULL	Application of aluminum	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Application of aluminum to the root cap strongly promoted acropetal transport of auxin reducing polarity from 6.3 to 2.1 .
	manualset3
240677	2	423622	15	NULL	NULL	0	NULL	root cap 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of aluminum to the root cap strongly promoted acropetal transport of auxin reducing polarity from 6.3 to 2.1 .
	manualset3
240678	3	423622	15	NULL	NULL	0	NULL	acropetal transport of auxin	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of aluminum to the root cap strongly promoted acropetal transport of auxin reducing polarity from 6.3 to 2.1 .
	manualset3
240679	4	423622	15	NULL	NULL	NULL	NULL	polarity	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Application of aluminum to the root cap strongly promoted acropetal transport of auxin reducing polarity from 6.3 to 2.1 .
	manualset3
258730	5	423622	15	NULL	NULL	NULL	NULL	6.3 to 2.1	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Application of aluminum to the root cap strongly promoted acropetal transport of auxin reducing polarity from 6.3 to 2.1 .
	manualset3
240774	1	423623	15	NULL	NULL	0	NULL	Application of ivabradine	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of ivabradine in these conditions deserves full attention , with dedicated and properly powered outcome trials .
	manualset3
240775	2	423623	15	NULL	NULL	0	NULL	conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of ivabradine in these conditions deserves full attention , with dedicated and properly powered outcome trials .
	manualset3
240776	3	423623	15	NULL	NULL	NULL	NULL	attention 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Application of ivabradine in these conditions deserves full attention , with dedicated and properly powered outcome trials .
	manualset3
240778	4	423623	15	NULL	NULL	0	NULL	dedicated outcome trials	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of ivabradine in these conditions deserves full attention , with dedicated and properly powered outcome trials .
	manualset3
240779	5	423623	15	NULL	NULL	0	NULL	properly powered outcome trials	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of ivabradine in these conditions deserves full attention , with dedicated and properly powered outcome trials .
	manualset3
240783	1	423624	15	NULL	NULL	0	NULL	Application of laser capture microdissection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of laser capture microdissection and proteomics in colon cancer .
	manualset3
240785	2	423624	15	NULL	NULL	0	NULL	 proteomics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of laser capture microdissection and proteomics in colon cancer .
	manualset3
240786	3	423624	15	NULL	NULL	0	NULL	colon cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of laser capture microdissection and proteomics in colon cancer .
	manualset3
240787	1	423625	15	NULL	NULL	0	NULL	Application of matrix metalloproteinase models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of matrix metalloproteinase models to migraine helps explain the ability of medications to cross the blood-brain barrier during a migraine episode , as well as describe possible ischemia with repeated migraine ( e.g. , white matter abnormalities seen on magnetic resonance scanning ) .
	manualset3
240788	2	423625	15	NULL	NULL	0	NULL	migraine	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of matrix metalloproteinase models to migraine helps explain the ability of medications to cross the blood-brain barrier during a migraine episode , as well as describe possible ischemia with repeated migraine ( e.g. , white matter abnormalities seen on magnetic resonance scanning ) .
	manualset3
240790	3	423625	15	NULL	NULL	0	NULL	ability of medications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of matrix metalloproteinase models to migraine helps explain the ability of medications to cross the blood-brain barrier during a migraine episode , as well as describe possible ischemia with repeated migraine ( e.g. , white matter abnormalities seen on magnetic resonance scanning ) .
	manualset3
240791	4	423625	15	NULL	NULL	0	NULL	blood-brain barrier	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of matrix metalloproteinase models to migraine helps explain the ability of medications to cross the blood-brain barrier during a migraine episode , as well as describe possible ischemia with repeated migraine ( e.g. , white matter abnormalities seen on magnetic resonance scanning ) .
	manualset3
240792	5	423625	15	NULL	NULL	0	NULL	migraine episode	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of matrix metalloproteinase models to migraine helps explain the ability of medications to cross the blood-brain barrier during a migraine episode , as well as describe possible ischemia with repeated migraine ( e.g. , white matter abnormalities seen on magnetic resonance scanning ) .
	manualset3
240793	6	423625	15	NULL	NULL	0	NULL	ischemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of matrix metalloproteinase models to migraine helps explain the ability of medications to cross the blood-brain barrier during a migraine episode , as well as describe possible ischemia with repeated migraine ( e.g. , white matter abnormalities seen on magnetic resonance scanning ) .
	manualset3
240794	7	423625	15	NULL	NULL	0	NULL	migraine	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of matrix metalloproteinase models to migraine helps explain the ability of medications to cross the blood-brain barrier during a migraine episode , as well as describe possible ischemia with repeated migraine ( e.g. , white matter abnormalities seen on magnetic resonance scanning ) .
	manualset3
240795	8	423625	15	NULL	NULL	0	NULL	white matter abnormalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of matrix metalloproteinase models to migraine helps explain the ability of medications to cross the blood-brain barrier during a migraine episode , as well as describe possible ischemia with repeated migraine ( e.g. , white matter abnormalities seen on magnetic resonance scanning ) .
	manualset3
240796	9	423625	15	NULL	NULL	0	NULL	magnetic resonance scanning	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of matrix metalloproteinase models to migraine helps explain the ability of medications to cross the blood-brain barrier during a migraine episode , as well as describe possible ischemia with repeated migraine ( e.g. , white matter abnormalities seen on magnetic resonance scanning ) .
	manualset3
240799	1	423626	15	NULL	NULL	0	NULL	Application of normal saline	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of normal saline to ultrasonography as an alternative to gel for internal jugular venous cannulation .
	manualset3
240801	2	423626	15	NULL	NULL	0	NULL	ultrasonography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of normal saline to ultrasonography as an alternative to gel for internal jugular venous cannulation .
	manualset3
240802	3	423626	15	NULL	NULL	NULL	NULL	gel	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Application of normal saline to ultrasonography as an alternative to gel for internal jugular venous cannulation .
	manualset3
240806	4	423626	15	NULL	NULL	0	NULL	internal jugular venous cannulation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of normal saline to ultrasonography as an alternative to gel for internal jugular venous cannulation .
	manualset3
240811	1	423627	15	NULL	NULL	0	NULL	Application of surface enhanced Raman spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of surface enhanced Raman spectroscopy to the study of SOFC electrode surfaces .
	manualset3
240812	2	423627	15	NULL	NULL	0	NULL	study of SOFC electrode surfaces	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of surface enhanced Raman spectroscopy to the study of SOFC electrode surfaces .
	manualset3
240815	1	423628	15	NULL	NULL	0	NULL	Application of the electrode	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of the electrode was attempted in 15 consecutive pregnancies .
	manualset3
240817	2	423628	15	NULL	NULL	0	NULL	15 consecutive pregnancies 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of the electrode was attempted in 15 consecutive pregnancies .
	manualset3
240822	1	423629	15	NULL	NULL	0	NULL	Application of the method	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of the method to plasma , blood and urine samples is presented .
	manualset3
240824	2	423629	15	NULL	NULL	NULL	NULL	plasma samples	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Application of the method to plasma , blood and urine samples is presented .
	manualset3
240825	3	423629	15	NULL	NULL	NULL	NULL	blood samples	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Application of the method to plasma , blood and urine samples is presented .
	manualset3
240826	4	423629	15	NULL	NULL	NULL	NULL	urine samples	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Application of the method to plasma , blood and urine samples is presented .
	manualset3
240828	1	423630	15	NULL	NULL	0	NULL	Effect of a sulfur-containing nucleotide-peptide complex	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of a sulfur-containing nucleotide-peptide complex on the growth and development of different species of algae ) .
	manualset3
240829	2	423630	15	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of a sulfur-containing nucleotide-peptide complex on the growth and development of different species of algae ) .
	manualset3
240830	3	423630	15	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of a sulfur-containing nucleotide-peptide complex on the growth and development of different species of algae ) .
	manualset3
240832	4	423630	15	NULL	NULL	NULL	NULL	species of algae 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Effect of a sulfur-containing nucleotide-peptide complex on the growth and development of different species of algae ) .
	manualset3
240892	1	423631	15	NULL	NULL	0	NULL	Application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of the participatory evaluation measurement index indicated the evaluation qualified as participatory at a minimal level historically and increased to a moderate level of participation after a re-design to involve an external evaluator .
	manualset3
240895	2	423631	15	NULL	NULL	0	NULL	participatory evaluation measurement index	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of the participatory evaluation measurement index indicated the evaluation qualified as participatory at a minimal level historically and increased to a moderate level of participation after a re-design to involve an external evaluator .
	manualset3
240896	3	423631	15	NULL	NULL	0	NULL	evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of the participatory evaluation measurement index indicated the evaluation qualified as participatory at a minimal level historically and increased to a moderate level of participation after a re-design to involve an external evaluator .
	manualset3
240905	4	423631	15	NULL	NULL	NULL	NULL	minimal level 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Application of the participatory evaluation measurement index indicated the evaluation qualified as participatory at a minimal level historically and increased to a moderate level of participation after a re-design to involve an external evaluator .
	manualset3
240906	5	423631	15	NULL	NULL	NULL	NULL	moderate level of participation 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Application of the participatory evaluation measurement index indicated the evaluation qualified as participatory at a minimal level historically and increased to a moderate level of participation after a re-design to involve an external evaluator .
	manualset3
240908	6	423631	15	NULL	NULL	0	NULL	re-design 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of the participatory evaluation measurement index indicated the evaluation qualified as participatory at a minimal level historically and increased to a moderate level of participation after a re-design to involve an external evaluator .
	manualset3
240909	7	423631	15	NULL	NULL	0	NULL	external evaluator	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of the participatory evaluation measurement index indicated the evaluation qualified as participatory at a minimal level historically and increased to a moderate level of participation after a re-design to involve an external evaluator .
	manualset3
240920	1	423632	15	NULL	NULL	0	NULL	Application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of two STRs ( VWA and TPO ) to human population profiling : survey in Galicia .
	manualset3
240922	2	423632	15	NULL	NULL	0	NULL	two STRs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of two STRs ( VWA and TPO ) to human population profiling : survey in Galicia .
	manualset3
240923	3	423632	15	NULL	NULL	0	NULL	VWA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of two STRs ( VWA and TPO ) to human population profiling : survey in Galicia .
	manualset3
240925	4	423632	15	NULL	NULL	0	NULL	TPO	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of two STRs ( VWA and TPO ) to human population profiling : survey in Galicia .
	manualset3
240926	5	423632	15	NULL	NULL	NULL	NULL	human population profiling	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Application of two STRs ( VWA and TPO ) to human population profiling : survey in Galicia .
	manualset3
240929	6	423632	15	NULL	NULL	NULL	NULL	survey	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Application of two STRs ( VWA and TPO ) to human population profiling : survey in Galicia .
	manualset3
240931	7	423632	15	NULL	NULL	0	NULL	Galicia	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Application of two STRs ( VWA and TPO ) to human population profiling : survey in Galicia .
	manualset3
240932	1	423633	15	NULL	NULL	0	NULL	Applications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Applications include the small-angle scattering , diffraction and absorption spectroscopy of lithium manganese oxide electrodes .
	manualset3
240933	2	423633	15	NULL	NULL	0	NULL	small-angle scattering	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Applications include the small-angle scattering , diffraction and absorption spectroscopy of lithium manganese oxide electrodes .
	manualset3
240934	3	423633	15	NULL	NULL	0	NULL	diffraction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Applications include the small-angle scattering , diffraction and absorption spectroscopy of lithium manganese oxide electrodes .
	manualset3
240935	4	423633	15	NULL	NULL	0	NULL	absorption spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Applications include the small-angle scattering , diffraction and absorption spectroscopy of lithium manganese oxide electrodes .
	manualset3
240936	5	423633	15	NULL	NULL	NULL	NULL	lithium manganese oxide	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Applications include the small-angle scattering , diffraction and absorption spectroscopy of lithium manganese oxide electrodes .
	manualset3
241935	6	423633	15	NULL	NULL	0	NULL	electrodes 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Applications include the small-angle scattering , diffraction and absorption spectroscopy of lithium manganese oxide electrodes .
	manualset3
240937	1	423634	15	NULL	NULL	0	NULL	Applications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Applications to alkanes , tryptophan , and polyglycine are presented .
	manualset3
240938	2	423634	15	NULL	NULL	0	NULL	alkanes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Applications to alkanes , tryptophan , and polyglycine are presented .
	manualset3
240939	3	423634	15	NULL	NULL	0	NULL	tryptophan	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Applications to alkanes , tryptophan , and polyglycine are presented .
	manualset3
240940	4	423634	15	NULL	NULL	NULL	NULL	polyglycine	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Applications to alkanes , tryptophan , and polyglycine are presented .
	manualset3
240941	1	423635	15	NULL	NULL	0	NULL	Applying multivariate analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Applying multivariate analysis , epidermoid cell type , even if exclusively for N2 tumors , was an independent prognostic factor , showing a favorable impact on survival expectancy ( 27.8 % at 90 months ) .
	manualset3
240942	2	423635	15	NULL	NULL	0	NULL	epidermoid cell type	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Applying multivariate analysis , epidermoid cell type , even if exclusively for N2 tumors , was an independent prognostic factor , showing a favorable impact on survival expectancy ( 27.8 % at 90 months ) .
	manualset3
240943	3	423635	15	NULL	NULL	0	NULL	N2 tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Applying multivariate analysis , epidermoid cell type , even if exclusively for N2 tumors , was an independent prognostic factor , showing a favorable impact on survival expectancy ( 27.8 % at 90 months ) .
	manualset3
240944	4	423635	15	NULL	NULL	0	NULL	independent prognostic factor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Applying multivariate analysis , epidermoid cell type , even if exclusively for N2 tumors , was an independent prognostic factor , showing a favorable impact on survival expectancy ( 27.8 % at 90 months ) .
	manualset3
240945	5	423635	15	NULL	NULL	0	NULL	favorable impact	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Applying multivariate analysis , epidermoid cell type , even if exclusively for N2 tumors , was an independent prognostic factor , showing a favorable impact on survival expectancy ( 27.8 % at 90 months ) .
	manualset3
240946	6	423635	15	NULL	NULL	0	NULL	survival expectancy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Applying multivariate analysis , epidermoid cell type , even if exclusively for N2 tumors , was an independent prognostic factor , showing a favorable impact on survival expectancy ( 27.8 % at 90 months ) .
	manualset3
240947	7	423635	15	NULL	NULL	0	NULL	27.8 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Applying multivariate analysis , epidermoid cell type , even if exclusively for N2 tumors , was an independent prognostic factor , showing a favorable impact on survival expectancy ( 27.8 % at 90 months ) .
	manualset3
240948	8	423635	15	NULL	NULL	0	NULL	90 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Applying multivariate analysis , epidermoid cell type , even if exclusively for N2 tumors , was an independent prognostic factor , showing a favorable impact on survival expectancy ( 27.8 % at 90 months ) .
	manualset3
240949	1	423636	15	NULL	NULL	0	NULL	Approaches	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Approaches to reduce both oxidative processes could focus on minimizing oxidising agents in meat .
	manualset3
240950	2	423636	15	NULL	NULL	0	NULL	oxidative processes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Approaches to reduce both oxidative processes could focus on minimizing oxidising agents in meat .
	manualset3
240951	3	423636	15	NULL	NULL	0	NULL	oxidising agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Approaches to reduce both oxidative processes could focus on minimizing oxidising agents in meat .
	manualset3
240952	4	423636	15	NULL	NULL	0	NULL	meat	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Approaches to reduce both oxidative processes could focus on minimizing oxidising agents in meat .
	manualset3
240953	1	423637	15	NULL	NULL	0	NULL	use of imaging biomarkers	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Appropriate use of imaging biomarkers -- defined as anatomic , physiologic , biochemical , or molecular parameters detectable with imaging methods used to establish the presence or severity of disease -- offer the prospect of smaller , less expensive , and more efficient preclinical studies and clinical trials .
	manualset3
240954	2	423637	15	NULL	NULL	0	NULL	anatomic parameters	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Appropriate use of imaging biomarkers -- defined as anatomic , physiologic , biochemical , or molecular parameters detectable with imaging methods used to establish the presence or severity of disease -- offer the prospect of smaller , less expensive , and more efficient preclinical studies and clinical trials .
	manualset3
240955	3	423637	15	NULL	NULL	0	NULL	physiologic parameters	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Appropriate use of imaging biomarkers -- defined as anatomic , physiologic , biochemical , or molecular parameters detectable with imaging methods used to establish the presence or severity of disease -- offer the prospect of smaller , less expensive , and more efficient preclinical studies and clinical trials .
	manualset3
240956	4	423637	15	NULL	NULL	0	NULL	biochemical parameters	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Appropriate use of imaging biomarkers -- defined as anatomic , physiologic , biochemical , or molecular parameters detectable with imaging methods used to establish the presence or severity of disease -- offer the prospect of smaller , less expensive , and more efficient preclinical studies and clinical trials .
	manualset3
240957	5	423637	15	NULL	NULL	0	NULL	molecular parameters	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Appropriate use of imaging biomarkers -- defined as anatomic , physiologic , biochemical , or molecular parameters detectable with imaging methods used to establish the presence or severity of disease -- offer the prospect of smaller , less expensive , and more efficient preclinical studies and clinical trials .
	manualset3
240958	6	423637	15	NULL	NULL	0	NULL	imaging methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Appropriate use of imaging biomarkers -- defined as anatomic , physiologic , biochemical , or molecular parameters detectable with imaging methods used to establish the presence or severity of disease -- offer the prospect of smaller , less expensive , and more efficient preclinical studies and clinical trials .
	manualset3
240959	7	423637	15	NULL	NULL	0	NULL	presence of disease	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Appropriate use of imaging biomarkers -- defined as anatomic , physiologic , biochemical , or molecular parameters detectable with imaging methods used to establish the presence or severity of disease -- offer the prospect of smaller , less expensive , and more efficient preclinical studies and clinical trials .
	manualset3
240961	8	423637	15	NULL	NULL	0	NULL	severity of disease 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Appropriate use of imaging biomarkers -- defined as anatomic , physiologic , biochemical , or molecular parameters detectable with imaging methods used to establish the presence or severity of disease -- offer the prospect of smaller , less expensive , and more efficient preclinical studies and clinical trials .
	manualset3
240962	9	423637	15	NULL	NULL	0	NULL	prospect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Appropriate use of imaging biomarkers -- defined as anatomic , physiologic , biochemical , or molecular parameters detectable with imaging methods used to establish the presence or severity of disease -- offer the prospect of smaller , less expensive , and more efficient preclinical studies and clinical trials .
	manualset3
240966	10	423637	15	NULL	NULL	0	NULL	preclinical studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Appropriate use of imaging biomarkers -- defined as anatomic , physiologic , biochemical , or molecular parameters detectable with imaging methods used to establish the presence or severity of disease -- offer the prospect of smaller , less expensive , and more efficient preclinical studies and clinical trials .
	manualset3
240968	11	423637	15	NULL	NULL	0	NULL	clinical trials 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Appropriate use of imaging biomarkers -- defined as anatomic , physiologic , biochemical , or molecular parameters detectable with imaging methods used to establish the presence or severity of disease -- offer the prospect of smaller , less expensive , and more efficient preclinical studies and clinical trials .
	manualset3
240978	1	423638	15	NULL	NULL	0	NULL	 Effect of dexamethasone	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of dexamethasone on skin phospholipid spectrum in laboratory animals ) .
	manualset3
240979	2	423638	15	NULL	NULL	0	NULL	skin phospholipid spectrum	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of dexamethasone on skin phospholipid spectrum in laboratory animals ) .
	manualset3
240980	3	423638	15	NULL	NULL	0	NULL	laboratory animals	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of dexamethasone on skin phospholipid spectrum in laboratory animals ) .
	manualset3
240986	1	423639	15	NULL	NULL	NULL	NULL	volumes	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Appropriate volumes of 2 % ( w/v ) calcium chloride solution were added to 0.4-2 mg/ml ceftriaxone isotonic sodium chloride solution , to make solutions with a final calcium ion concentration of 1.25 mmol/l .
	manualset3
240988	3	423639	15	NULL	NULL	NULL	NULL	calcium chloride solution	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Appropriate volumes of 2 % ( w/v ) calcium chloride solution were added to 0.4-2 mg/ml ceftriaxone isotonic sodium chloride solution , to make solutions with a final calcium ion concentration of 1.25 mmol/l .
	manualset3
240991	4	423639	15	NULL	NULL	NULL	NULL	0.4-2 mg/ml 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Appropriate volumes of 2 % ( w/v ) calcium chloride solution were added to 0.4-2 mg/ml ceftriaxone isotonic sodium chloride solution , to make solutions with a final calcium ion concentration of 1.25 mmol/l .
	manualset3
240992	5	423639	15	NULL	NULL	NULL	NULL	ceftriaxone isotonic sodium chloride solution	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Appropriate volumes of 2 % ( w/v ) calcium chloride solution were added to 0.4-2 mg/ml ceftriaxone isotonic sodium chloride solution , to make solutions with a final calcium ion concentration of 1.25 mmol/l .
	manualset3
240993	6	423639	15	NULL	NULL	NULL	NULL	solutions	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Appropriate volumes of 2 % ( w/v ) calcium chloride solution were added to 0.4-2 mg/ml ceftriaxone isotonic sodium chloride solution , to make solutions with a final calcium ion concentration of 1.25 mmol/l .
	manualset3
240994	7	423639	15	NULL	NULL	NULL	NULL	calcium ion concentration 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Appropriate volumes of 2 % ( w/v ) calcium chloride solution were added to 0.4-2 mg/ml ceftriaxone isotonic sodium chloride solution , to make solutions with a final calcium ion concentration of 1.25 mmol/l .
	manualset3
258751	2	423639	15	NULL	NULL	NULL	NULL	2 % ( w/v )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Appropriate volumes of 2 % ( w/v ) calcium chloride solution were added to 0.4-2 mg/ml ceftriaxone isotonic sodium chloride solution , to make solutions with a final calcium ion concentration of 1.25 mmol/l .
	manualset3
258752	8	423639	15	NULL	NULL	NULL	NULL	1.25 mmol/l 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Appropriate volumes of 2 % ( w/v ) calcium chloride solution were added to 0.4-2 mg/ml ceftriaxone isotonic sodium chloride solution , to make solutions with a final calcium ion concentration of 1.25 mmol/l .
	manualset3
240995	1	423640	15	NULL	NULL	0	NULL	educational efforts 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Appropriately targeted educational efforts are needed to limit HIV transmission among adolescents .
	manualset3
240996	2	423640	15	NULL	NULL	0	NULL	HIV transmission	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Appropriately targeted educational efforts are needed to limit HIV transmission among adolescents .
	manualset3
240997	3	423640	15	NULL	NULL	0	NULL	adolescents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Appropriately targeted educational efforts are needed to limit HIV transmission among adolescents .
	manualset3
240998	1	423641	15	NULL	NULL	0	NULL	1 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 1 % of the orally administered dose was eliminated in urine as DMP .
	manualset3
240999	2	423641	15	NULL	NULL	0	NULL	orally administered dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 1 % of the orally administered dose was eliminated in urine as DMP .
	manualset3
241000	3	423641	15	NULL	NULL	0	NULL	urine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 1 % of the orally administered dose was eliminated in urine as DMP .
	manualset3
241001	4	423641	15	NULL	NULL	0	NULL	DMP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 1 % of the orally administered dose was eliminated in urine as DMP .
	manualset3
241002	1	423642	15	NULL	NULL	0	NULL	15-40 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 15-40 % higher densities of ( 3H ) 8-OH-DPAT binding were observed in the anterior cortical regions of the periadolescent P rat compared with NP rat pups .
	manualset3
241004	2	423642	15	NULL	NULL	0	NULL	densities 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 15-40 % higher densities of ( 3H ) 8-OH-DPAT binding were observed in the anterior cortical regions of the periadolescent P rat compared with NP rat pups .
	manualset3
241007	3	423642	15	NULL	NULL	0	NULL	( 3H ) 8-OH-DPAT binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 15-40 % higher densities of ( 3H ) 8-OH-DPAT binding were observed in the anterior cortical regions of the periadolescent P rat compared with NP rat pups .
	manualset3
241009	4	423642	15	NULL	NULL	0	NULL	anterior cortical regions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 15-40 % higher densities of ( 3H ) 8-OH-DPAT binding were observed in the anterior cortical regions of the periadolescent P rat compared with NP rat pups .
	manualset3
241011	5	423642	15	NULL	NULL	0	NULL	periadolescent P rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 15-40 % higher densities of ( 3H ) 8-OH-DPAT binding were observed in the anterior cortical regions of the periadolescent P rat compared with NP rat pups .
	manualset3
241014	6	423642	15	NULL	NULL	0	NULL	NP rat pups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 15-40 % higher densities of ( 3H ) 8-OH-DPAT binding were observed in the anterior cortical regions of the periadolescent P rat compared with NP rat pups .
	manualset3
241019	1	423643	15	NULL	NULL	0	NULL	15 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 15 % of adult background hprt mutations are due to gross structural alterations ( primarily deletions ) having random breakpoints ; 85 % result from `` point '' changes detected only by sequencing .
	manualset3
241020	2	423643	15	NULL	NULL	0	NULL	adult background hprt mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 15 % of adult background hprt mutations are due to gross structural alterations ( primarily deletions ) having random breakpoints ; 85 % result from `` point '' changes detected only by sequencing .
	manualset3
241022	3	423643	15	NULL	NULL	0	NULL	gross structural alterations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 15 % of adult background hprt mutations are due to gross structural alterations ( primarily deletions ) having random breakpoints ; 85 % result from `` point '' changes detected only by sequencing .
	manualset3
241023	4	423643	15	NULL	NULL	0	NULL	primarily deletions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 15 % of adult background hprt mutations are due to gross structural alterations ( primarily deletions ) having random breakpoints ; 85 % result from `` point '' changes detected only by sequencing .
	manualset3
241027	5	423643	15	NULL	NULL	0	NULL	random breakpoints	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 15 % of adult background hprt mutations are due to gross structural alterations ( primarily deletions ) having random breakpoints ; 85 % result from `` point '' changes detected only by sequencing .
	manualset3
241028	6	423643	15	NULL	NULL	0	NULL	85 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 15 % of adult background hprt mutations are due to gross structural alterations ( primarily deletions ) having random breakpoints ; 85 % result from `` point '' changes detected only by sequencing .
	manualset3
241029	7	423643	15	NULL	NULL	0	NULL	`` point '' changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 15 % of adult background hprt mutations are due to gross structural alterations ( primarily deletions ) having random breakpoints ; 85 % result from `` point '' changes detected only by sequencing .
	manualset3
241030	8	423643	15	NULL	NULL	0	NULL	sequencing	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 15 % of adult background hprt mutations are due to gross structural alterations ( primarily deletions ) having random breakpoints ; 85 % result from `` point '' changes detected only by sequencing .
	manualset3
241031	1	423644	15	NULL	NULL	0	NULL	20 % ( 10/48 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 20 % ( 10/48 ) , however , demonstrated abnormal acid exposure ( total time pH & lt ; 4.0 , 18.8 + / - 14.8 % ) .
	manualset3
241032	2	423644	15	NULL	NULL	0	NULL	abnormal acid exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 20 % ( 10/48 ) , however , demonstrated abnormal acid exposure ( total time pH & lt ; 4.0 , 18.8 + / - 14.8 % ) .
	manualset3
241033	3	423644	15	NULL	NULL	0	NULL	total time pH & lt ; 4.0 , 18.8 + / - 14.8 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 20 % ( 10/48 ) , however , demonstrated abnormal acid exposure ( total time pH & lt ; 4.0 , 18.8 + / - 14.8 % ) .
	manualset3
241036	1	423645	15	NULL	NULL	0	NULL	5 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 5 % of the nerve fibers reach the ipsilateral optic tectum ( IOT ) via the ipsilateral tract at the chiasma .
	manualset3
241046	2	423645	15	NULL	NULL	0	NULL	nerve fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 5 % of the nerve fibers reach the ipsilateral optic tectum ( IOT ) via the ipsilateral tract at the chiasma .
	manualset3
241048	3	423645	15	NULL	NULL	0	NULL	ipsilateral optic tectum ( IOT ) 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 5 % of the nerve fibers reach the ipsilateral optic tectum ( IOT ) via the ipsilateral tract at the chiasma .
	manualset3
241050	4	423645	15	NULL	NULL	0	NULL	ipsilateral tract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 5 % of the nerve fibers reach the ipsilateral optic tectum ( IOT ) via the ipsilateral tract at the chiasma .
	manualset3
241051	5	423645	15	NULL	NULL	0	NULL	chiasma	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 5 % of the nerve fibers reach the ipsilateral optic tectum ( IOT ) via the ipsilateral tract at the chiasma .
	manualset3
241054	1	423646	15	NULL	NULL	0	NULL	60 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 60 % of SOM cells in these nuclei expressed AR immunoreactivity in the male while significantly ( P & lt ; 0.01 ) fewer did so in the female ( approximately 25 % ) .
	manualset3
241056	2	423646	15	NULL	NULL	0	NULL	SOM cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 60 % of SOM cells in these nuclei expressed AR immunoreactivity in the male while significantly ( P & lt ; 0.01 ) fewer did so in the female ( approximately 25 % ) .
	manualset3
241057	3	423646	15	NULL	NULL	0	NULL	 nuclei	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 60 % of SOM cells in these nuclei expressed AR immunoreactivity in the male while significantly ( P & lt ; 0.01 ) fewer did so in the female ( approximately 25 % ) .
	manualset3
241058	4	423646	15	NULL	NULL	0	NULL	AR immunoreactivity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 60 % of SOM cells in these nuclei expressed AR immunoreactivity in the male while significantly ( P & lt ; 0.01 ) fewer did so in the female ( approximately 25 % ) .
	manualset3
241059	5	423646	15	NULL	NULL	0	NULL	male	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 60 % of SOM cells in these nuclei expressed AR immunoreactivity in the male while significantly ( P & lt ; 0.01 ) fewer did so in the female ( approximately 25 % ) .
	manualset3
241060	6	423646	15	NULL	NULL	0	NULL	P & lt ; 0.01	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 60 % of SOM cells in these nuclei expressed AR immunoreactivity in the male while significantly ( P & lt ; 0.01 ) fewer did so in the female ( approximately 25 % ) .
	manualset3
241062	7	423646	15	NULL	NULL	0	NULL	female	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 60 % of SOM cells in these nuclei expressed AR immunoreactivity in the male while significantly ( P & lt ; 0.01 ) fewer did so in the female ( approximately 25 % ) .
	manualset3
241064	8	423646	15	NULL	NULL	NULL	NULL	25 % 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Approximately 60 % of SOM cells in these nuclei expressed AR immunoreactivity in the male while significantly ( P & lt ; 0.01 ) fewer did so in the female ( approximately 25 % ) .
	manualset3
241067	1	423647	15	NULL	NULL	0	NULL	600 U/h 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 600 U/h of heparin were given to increase aPTT to approximately 60 s. Plasma levels of all adhesion molecules increased in all groups .
	manualset3
241068	2	423647	15	NULL	NULL	0	NULL	heparin 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 600 U/h of heparin were given to increase aPTT to approximately 60 s. Plasma levels of all adhesion molecules increased in all groups .
	manualset3
241071	3	423647	15	NULL	NULL	NULL	NULL	aPTT	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Approximately 600 U/h of heparin were given to increase aPTT to approximately 60 s. Plasma levels of all adhesion molecules increased in all groups .
	manualset3
241072	4	423647	15	NULL	NULL	0	NULL	60 s	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 600 U/h of heparin were given to increase aPTT to approximately 60 s. Plasma levels of all adhesion molecules increased in all groups .
	manualset3
241076	5	423647	15	NULL	NULL	0	NULL	Plasma levels of all adhesion molecules	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 600 U/h of heparin were given to increase aPTT to approximately 60 s. Plasma levels of all adhesion molecules increased in all groups .
	manualset3
241078	6	423647	15	NULL	NULL	0	NULL	groups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 600 U/h of heparin were given to increase aPTT to approximately 60 s. Plasma levels of all adhesion molecules increased in all groups .
	manualset3
241085	1	423648	15	NULL	NULL	0	NULL	Effect of diets	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of diets with different caloric levels on blood protein turnover ) .
	manualset3
241087	2	423648	15	NULL	NULL	0	NULL	caloric levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of diets with different caloric levels on blood protein turnover ) .
	manualset3
241089	3	423648	15	NULL	NULL	0	NULL	blood protein turnover	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of diets with different caloric levels on blood protein turnover ) .
	manualset3
241091	1	423649	15	NULL	NULL	0	NULL	70 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 70 % of the participants reported that media ( TV and/or radio ) was the source of their information .
	manualset3
241093	2	423649	15	NULL	NULL	0	NULL	participants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 70 % of the participants reported that media ( TV and/or radio ) was the source of their information .
	manualset3
241096	3	423649	15	NULL	NULL	0	NULL	media	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 70 % of the participants reported that media ( TV and/or radio ) was the source of their information .
	manualset3
241097	4	423649	15	NULL	NULL	0	NULL	TV 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 70 % of the participants reported that media ( TV and/or radio ) was the source of their information .
	manualset3
241099	5	423649	15	NULL	NULL	0	NULL	radio	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 70 % of the participants reported that media ( TV and/or radio ) was the source of their information .
	manualset3
241102	6	423649	15	NULL	NULL	0	NULL	source of their information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Approximately 70 % of the participants reported that media ( TV and/or radio ) was the source of their information .
	manualset3
241105	1	423650	15	NULL	NULL	0	NULL	Aprotinin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Aprotinin at 50 to 200 kallikrein inhibiting units/mL decreased the expression of activated GP IIb-IIIa complex in response to adenosine diphosphate or thrombin receptor activator peptide 6 in a dose-dependent manner in both citrated and heparinized whole blood experiments .
	manualset3
241106	2	423650	15	NULL	NULL	0	NULL	50 to 200 kallikrein inhibiting units/mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Aprotinin at 50 to 200 kallikrein inhibiting units/mL decreased the expression of activated GP IIb-IIIa complex in response to adenosine diphosphate or thrombin receptor activator peptide 6 in a dose-dependent manner in both citrated and heparinized whole blood experiments .
	manualset3
241244	3	423650	15	NULL	NULL	0	NULL	expression of activated GP IIb-IIIa complex 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Aprotinin at 50 to 200 kallikrein inhibiting units/mL decreased the expression of activated GP IIb-IIIa complex in response to adenosine diphosphate or thrombin receptor activator peptide 6 in a dose-dependent manner in both citrated and heparinized whole blood experiments .
	manualset3
241245	4	423650	15	NULL	NULL	0	NULL	response	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Aprotinin at 50 to 200 kallikrein inhibiting units/mL decreased the expression of activated GP IIb-IIIa complex in response to adenosine diphosphate or thrombin receptor activator peptide 6 in a dose-dependent manner in both citrated and heparinized whole blood experiments .
	manualset3
241246	5	423650	15	NULL	NULL	0	NULL	adenosine diphosphate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Aprotinin at 50 to 200 kallikrein inhibiting units/mL decreased the expression of activated GP IIb-IIIa complex in response to adenosine diphosphate or thrombin receptor activator peptide 6 in a dose-dependent manner in both citrated and heparinized whole blood experiments .
	manualset3
241247	6	423650	15	NULL	NULL	0	NULL	thrombin receptor activator peptide 6	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Aprotinin at 50 to 200 kallikrein inhibiting units/mL decreased the expression of activated GP IIb-IIIa complex in response to adenosine diphosphate or thrombin receptor activator peptide 6 in a dose-dependent manner in both citrated and heparinized whole blood experiments .
	manualset3
241248	7	423650	15	NULL	NULL	0	NULL	dose-dependent manner	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Aprotinin at 50 to 200 kallikrein inhibiting units/mL decreased the expression of activated GP IIb-IIIa complex in response to adenosine diphosphate or thrombin receptor activator peptide 6 in a dose-dependent manner in both citrated and heparinized whole blood experiments .
	manualset3
241249	8	423650	15	NULL	NULL	0	NULL	citrated blood experiments 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Aprotinin at 50 to 200 kallikrein inhibiting units/mL decreased the expression of activated GP IIb-IIIa complex in response to adenosine diphosphate or thrombin receptor activator peptide 6 in a dose-dependent manner in both citrated and heparinized whole blood experiments .
	manualset3
241250	9	423650	15	NULL	NULL	0	NULL	heparinized whole blood experiments 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Aprotinin at 50 to 200 kallikrein inhibiting units/mL decreased the expression of activated GP IIb-IIIa complex in response to adenosine diphosphate or thrombin receptor activator peptide 6 in a dose-dependent manner in both citrated and heparinized whole blood experiments .
	manualset3
241251	1	423651	15	NULL	NULL	0	NULL	Aptamer selection strategies	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Aptamer selection strategies , however , typically do not select for the conformation-switching architectures , and as such several approaches have been reported to date by which aptamers can be re-engineered such that they undergo the binding-induced switching required to support efficient E-AB signaling .
	manualset3
241252	2	423651	15	NULL	NULL	0	NULL	conformation-switching architectures	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Aptamer selection strategies , however , typically do not select for the conformation-switching architectures , and as such several approaches have been reported to date by which aptamers can be re-engineered such that they undergo the binding-induced switching required to support efficient E-AB signaling .
	manualset3
241253	3	423651	15	NULL	NULL	0	NULL	several approaches 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Aptamer selection strategies , however , typically do not select for the conformation-switching architectures , and as such several approaches have been reported to date by which aptamers can be re-engineered such that they undergo the binding-induced switching required to support efficient E-AB signaling .
	manualset3
241254	4	423651	15	NULL	NULL	0	NULL	aptamers 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Aptamer selection strategies , however , typically do not select for the conformation-switching architectures , and as such several approaches have been reported to date by which aptamers can be re-engineered such that they undergo the binding-induced switching required to support efficient E-AB signaling .
	manualset3
241255	5	423651	15	NULL	NULL	0	NULL	binding-induced switching 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Aptamer selection strategies , however , typically do not select for the conformation-switching architectures , and as such several approaches have been reported to date by which aptamers can be re-engineered such that they undergo the binding-induced switching required to support efficient E-AB signaling .
	manualset3
241256	6	423651	15	NULL	NULL	0	NULL	E-AB signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Aptamer selection strategies , however , typically do not select for the conformation-switching architectures , and as such several approaches have been reported to date by which aptamers can be re-engineered such that they undergo the binding-induced switching required to support efficient E-AB signaling .
	manualset3
241257	1	423652	15	NULL	NULL	0	NULL	Apurinic/apyrimidinic endonuclease 1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Apurinic/apyrimidinic endonuclease 1 , p53 , and thioredoxin are linked in control of aging in C. elegans .
	manualset3
241258	2	423652	15	NULL	NULL	0	NULL	p53	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Apurinic/apyrimidinic endonuclease 1 , p53 , and thioredoxin are linked in control of aging in C. elegans .
	manualset3
241259	3	423652	15	NULL	NULL	0	NULL	thioredoxin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Apurinic/apyrimidinic endonuclease 1 , p53 , and thioredoxin are linked in control of aging in C. elegans .
	manualset3
241260	4	423652	15	NULL	NULL	0	NULL	control of aging 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Apurinic/apyrimidinic endonuclease 1 , p53 , and thioredoxin are linked in control of aging in C. elegans .
	manualset3
241261	5	423652	15	NULL	NULL	0	NULL	C. elegans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Apurinic/apyrimidinic endonuclease 1 , p53 , and thioredoxin are linked in control of aging in C. elegans .
	manualset3
241262	1	423653	15	NULL	NULL	0	NULL	Aquaporin 5 ( Aqp5 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Aquaporin 5 ( Aqp5 ) , a member of the aquaporin family of membrane water channels , is thought to modulate the osmolality of fluids in the eye , lung , and salivary gland .
	manualset3
241263	2	423653	15	NULL	NULL	0	NULL	member	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Aquaporin 5 ( Aqp5 ) , a member of the aquaporin family of membrane water channels , is thought to modulate the osmolality of fluids in the eye , lung , and salivary gland .
	manualset3
241264	3	423653	15	NULL	NULL	0	NULL	aquaporin family of membrane water channels	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Aquaporin 5 ( Aqp5 ) , a member of the aquaporin family of membrane water channels , is thought to modulate the osmolality of fluids in the eye , lung , and salivary gland .
	manualset3
241265	4	423653	15	NULL	NULL	0	NULL	osmolality of fluids	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Aquaporin 5 ( Aqp5 ) , a member of the aquaporin family of membrane water channels , is thought to modulate the osmolality of fluids in the eye , lung , and salivary gland .
	manualset3
241266	5	423653	15	NULL	NULL	0	NULL	eye	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Aquaporin 5 ( Aqp5 ) , a member of the aquaporin family of membrane water channels , is thought to modulate the osmolality of fluids in the eye , lung , and salivary gland .
	manualset3
241267	6	423653	15	NULL	NULL	0	NULL	lung	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Aquaporin 5 ( Aqp5 ) , a member of the aquaporin family of membrane water channels , is thought to modulate the osmolality of fluids in the eye , lung , and salivary gland .
	manualset3
241268	7	423653	15	NULL	NULL	0	NULL	salivary gland	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Aquaporin 5 ( Aqp5 ) , a member of the aquaporin family of membrane water channels , is thought to modulate the osmolality of fluids in the eye , lung , and salivary gland .
	manualset3
241269	1	423654	15	NULL	NULL	NULL	NULL	Aqueous extract	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Aqueous extract of G. indica significantly decreased both the fasting and postprandial blood glucose in type 2 diabetic rats .
	manualset3
241270	3	423654	15	NULL	NULL	NULL	NULL	fasting blood glucose	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Aqueous extract of G. indica significantly decreased both the fasting and postprandial blood glucose in type 2 diabetic rats .
	manualset3
241271	4	423654	15	NULL	NULL	NULL	NULL	postprandial blood glucose 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Aqueous extract of G. indica significantly decreased both the fasting and postprandial blood glucose in type 2 diabetic rats .
	manualset3
241272	5	423654	15	NULL	NULL	NULL	NULL	type 2 diabetic rats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Aqueous extract of G. indica significantly decreased both the fasting and postprandial blood glucose in type 2 diabetic rats .
	manualset3
241936	2	423654	15	NULL	NULL	0	NULL	G. indica	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Aqueous extract of G. indica significantly decreased both the fasting and postprandial blood glucose in type 2 diabetic rats .
	manualset3
241273	1	423655	15	NULL	NULL	0	NULL	Effect of gestrinone	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of gestrinone on the lipid metabolic parameters and bone mineral density in patients with endometriosis ) .
	manualset3
241274	2	423655	15	NULL	NULL	0	NULL	lipid metabolic parameters 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of gestrinone on the lipid metabolic parameters and bone mineral density in patients with endometriosis ) .
	manualset3
241275	3	423655	15	NULL	NULL	0	NULL	bone mineral density	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of gestrinone on the lipid metabolic parameters and bone mineral density in patients with endometriosis ) .
	manualset3
241276	4	423655	15	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of gestrinone on the lipid metabolic parameters and bone mineral density in patients with endometriosis ) .
	manualset3
241277	5	423655	15	NULL	NULL	0	NULL	endometriosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of gestrinone on the lipid metabolic parameters and bone mineral density in patients with endometriosis ) .
	manualset3
241278	1	423656	15	NULL	NULL	0	NULL	Aqueous humor dynamics	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Aqueous humor dynamics in monkeys ( Macaca irus and Cercopithecus ethiops ) .
	manualset3
241279	2	423656	15	NULL	NULL	0	NULL	monkeys	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Aqueous humor dynamics in monkeys ( Macaca irus and Cercopithecus ethiops ) .
	manualset3
241280	3	423656	15	NULL	NULL	0	NULL	Macaca irus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Aqueous humor dynamics in monkeys ( Macaca irus and Cercopithecus ethiops ) .
	manualset3
241281	4	423656	15	NULL	NULL	0	NULL	Cercopithecus ethiops	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Aqueous humor dynamics in monkeys ( Macaca irus and Cercopithecus ethiops ) .
	manualset3
241282	1	423657	15	NULL	NULL	0	NULL	Ara-HxMP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ara-HxMP prevented hepatitis-associated deaths in hamsters , reduced the titer of EAV developing in hamsters , and inhibited the increase of serum glutamic pyruvic transaminase in EAV-infected hamsters .
	manualset3
241283	2	423657	15	NULL	NULL	0	NULL	hepatitis-associated deaths	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ara-HxMP prevented hepatitis-associated deaths in hamsters , reduced the titer of EAV developing in hamsters , and inhibited the increase of serum glutamic pyruvic transaminase in EAV-infected hamsters .
	manualset3
241284	3	423657	15	NULL	NULL	0	NULL	hamsters	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ara-HxMP prevented hepatitis-associated deaths in hamsters , reduced the titer of EAV developing in hamsters , and inhibited the increase of serum glutamic pyruvic transaminase in EAV-infected hamsters .
	manualset3
241285	4	423657	15	NULL	NULL	0	NULL	titer of EAV	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ara-HxMP prevented hepatitis-associated deaths in hamsters , reduced the titer of EAV developing in hamsters , and inhibited the increase of serum glutamic pyruvic transaminase in EAV-infected hamsters .
	manualset3
241286	5	423657	15	NULL	NULL	0	NULL	hamsters	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ara-HxMP prevented hepatitis-associated deaths in hamsters , reduced the titer of EAV developing in hamsters , and inhibited the increase of serum glutamic pyruvic transaminase in EAV-infected hamsters .
	manualset3
241287	6	423657	15	NULL	NULL	0	NULL	increase of serum glutamic pyruvic transaminase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ara-HxMP prevented hepatitis-associated deaths in hamsters , reduced the titer of EAV developing in hamsters , and inhibited the increase of serum glutamic pyruvic transaminase in EAV-infected hamsters .
	manualset3
241288	7	423657	15	NULL	NULL	0	NULL	EAV-infected hamsters	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Ara-HxMP prevented hepatitis-associated deaths in hamsters , reduced the titer of EAV developing in hamsters , and inhibited the increase of serum glutamic pyruvic transaminase in EAV-infected hamsters .
	manualset3
241289	1	423658	15	NULL	NULL	NULL	NULL	Arachidonic acids	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Arachidonic , oleic , linoleic , linolenic , and docosahexaenoic acids were active in this role , whereas saturated fatty acids such as palmitic and stearic acids were inactive .
	manualset3
241290	2	423658	15	NULL	NULL	NULL	NULL	oleic acids	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Arachidonic , oleic , linoleic , linolenic , and docosahexaenoic acids were active in this role , whereas saturated fatty acids such as palmitic and stearic acids were inactive .
	manualset3
241291	3	423658	15	NULL	NULL	NULL	NULL	linoleic acids 	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Arachidonic , oleic , linoleic , linolenic , and docosahexaenoic acids were active in this role , whereas saturated fatty acids such as palmitic and stearic acids were inactive .
	manualset3
241292	4	423658	15	NULL	NULL	NULL	NULL	linolenic acids 	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Arachidonic , oleic , linoleic , linolenic , and docosahexaenoic acids were active in this role , whereas saturated fatty acids such as palmitic and stearic acids were inactive .
	manualset3
241293	5	423658	15	NULL	NULL	NULL	NULL	docosahexaenoic acids	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Arachidonic , oleic , linoleic , linolenic , and docosahexaenoic acids were active in this role , whereas saturated fatty acids such as palmitic and stearic acids were inactive .
	manualset3
241294	6	423658	15	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Arachidonic , oleic , linoleic , linolenic , and docosahexaenoic acids were active in this role , whereas saturated fatty acids such as palmitic and stearic acids were inactive .
	manualset3
241295	7	423658	15	NULL	NULL	0	NULL	saturated fatty acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Arachidonic , oleic , linoleic , linolenic , and docosahexaenoic acids were active in this role , whereas saturated fatty acids such as palmitic and stearic acids were inactive .
	manualset3
241296	8	423658	15	NULL	NULL	0	NULL	palmitic acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Arachidonic , oleic , linoleic , linolenic , and docosahexaenoic acids were active in this role , whereas saturated fatty acids such as palmitic and stearic acids were inactive .
	manualset3
241297	9	423658	15	NULL	NULL	0	NULL	stearic acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Arachidonic , oleic , linoleic , linolenic , and docosahexaenoic acids were active in this role , whereas saturated fatty acids such as palmitic and stearic acids were inactive .
	manualset3
241298	1	423659	15	NULL	NULL	0	NULL	Arachidonic acid-induced IL-6 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Arachidonic acid-induced IL-6 expression is mediated by PKC alpha activation in osteoblastic cells .
	manualset3
241299	2	423659	15	NULL	NULL	0	NULL	PKC alpha activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Arachidonic acid-induced IL-6 expression is mediated by PKC alpha activation in osteoblastic cells .
	manualset3
241300	3	423659	15	NULL	NULL	0	NULL	osteoblastic cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Arachidonic acid-induced IL-6 expression is mediated by PKC alpha activation in osteoblastic cells .
	manualset3
241301	1	423660	15	NULL	NULL	0	NULL	Arachidonic acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Arachidonic and docosahexaenoic acids differentially affect the expression of fatty acyl-CoA oxidase , protein kinase C and lipid peroxidation in HepG2 cells .
	manualset3
241302	2	423660	15	NULL	NULL	0	NULL	docosahexaenoic acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Arachidonic and docosahexaenoic acids differentially affect the expression of fatty acyl-CoA oxidase , protein kinase C and lipid peroxidation in HepG2 cells .
	manualset3
241303	3	423660	15	NULL	NULL	0	NULL	expression of fatty acyl-CoA oxidase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Arachidonic and docosahexaenoic acids differentially affect the expression of fatty acyl-CoA oxidase , protein kinase C and lipid peroxidation in HepG2 cells .
	manualset3
241304	4	423660	15	NULL	NULL	0	NULL	protein kinase C peroxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Arachidonic and docosahexaenoic acids differentially affect the expression of fatty acyl-CoA oxidase , protein kinase C and lipid peroxidation in HepG2 cells .
	manualset3
241305	5	423660	15	NULL	NULL	0	NULL	lipid peroxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Arachidonic and docosahexaenoic acids differentially affect the expression of fatty acyl-CoA oxidase , protein kinase C and lipid peroxidation in HepG2 cells .
	manualset3
241306	6	423660	15	NULL	NULL	0	NULL	HepG2 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Arachidonic and docosahexaenoic acids differentially affect the expression of fatty acyl-CoA oxidase , protein kinase C and lipid peroxidation in HepG2 cells .
	manualset3
241307	1	423661	15	NULL	NULL	0	NULL	stress responses	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Are stress responses to geomagnetic storms mediated by the cryptochrome compass system ?
	manualset3
241308	2	423661	15	NULL	NULL	0	NULL	geomagnetic storms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Are stress responses to geomagnetic storms mediated by the cryptochrome compass system ?
	manualset3
241309	3	423661	15	NULL	NULL	0	NULL	cryptochrome compass system	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Are stress responses to geomagnetic storms mediated by the cryptochrome compass system ?
	manualset3
241310	1	423662	15	NULL	NULL	0	NULL	thyroid cancer patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Are thyroid cancer patients sensitive to ionising radiation ?
	manualset3
241311	2	423662	15	NULL	NULL	0	NULL	ionising radiation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Are thyroid cancer patients sensitive to ionising radiation ?
	manualset3
241312	1	423663	15	NULL	NULL	0	NULL	Effect of glycosylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of glycosylation on collagen type I fibrillogenesis in a model of connective tissue ) .
	manualset3
241313	2	423663	15	NULL	NULL	0	NULL	collagen type I fibrillogenesis 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of glycosylation on collagen type I fibrillogenesis in a model of connective tissue ) .
	manualset3
241314	3	423663	15	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of glycosylation on collagen type I fibrillogenesis in a model of connective tissue ) .
	manualset3
241315	4	423663	15	NULL	NULL	0	NULL	connective tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of glycosylation on collagen type I fibrillogenesis in a model of connective tissue ) .
	manualset3
241316	1	423664	15	NULL	NULL	0	NULL	Arene sulfonamides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Arene - and quinoline-sulfonamides as novel 5-HT7 receptor ligands .
	manualset3
241317	2	423664	15	NULL	NULL	0	NULL	quinoline-sulfonamides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Arene - and quinoline-sulfonamides as novel 5-HT7 receptor ligands .
	manualset3
241318	3	423664	15	NULL	NULL	NULL	NULL	5-HT7 receptor ligands	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Arene - and quinoline-sulfonamides as novel 5-HT7 receptor ligands .
	manualset3
241319	1	423665	15	NULL	NULL	0	NULL	Argatroban dosing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Argatroban dosing in intensive care patients with acute renal failure and liver dysfunction .
	manualset3
241320	2	423665	15	NULL	NULL	0	NULL	intensive care patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Argatroban dosing in intensive care patients with acute renal failure and liver dysfunction .
	manualset3
241321	3	423665	15	NULL	NULL	0	NULL	acute renal failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Argatroban dosing in intensive care patients with acute renal failure and liver dysfunction .
	manualset3
241322	4	423665	15	NULL	NULL	0	NULL	liver dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Argatroban dosing in intensive care patients with acute renal failure and liver dysfunction .
	manualset3
241323	1	423666	15	NULL	NULL	0	NULL	Arginine hydrochloride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Arginine hydrochloride has been used to suppress protein aggregation during refolding and in various other applications .
	manualset3
241324	2	423666	15	NULL	NULL	NULL	NULL	protein aggregation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Arginine hydrochloride has been used to suppress protein aggregation during refolding and in various other applications .
	manualset3
241325	3	423666	15	NULL	NULL	0	NULL	refolding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Arginine hydrochloride has been used to suppress protein aggregation during refolding and in various other applications .
	manualset3
241326	4	423666	15	NULL	NULL	0	NULL	applications	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Arginine hydrochloride has been used to suppress protein aggregation during refolding and in various other applications .
	manualset3
241327	1	423667	15	NULL	NULL	0	NULL	Arguments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Arguments against 5-hydroxytryptamine as neurotransmitter in the rabbit retina .
	manualset3
241328	2	423667	15	NULL	NULL	0	NULL	 5-hydroxytryptamine 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Arguments against 5-hydroxytryptamine as neurotransmitter in the rabbit retina .
	manualset3
241329	3	423667	15	NULL	NULL	0	NULL	neurotransmitter 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Arguments against 5-hydroxytryptamine as neurotransmitter in the rabbit retina .
	manualset3
241330	4	423667	15	NULL	NULL	0	NULL	rabbit retina	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Arguments against 5-hydroxytryptamine as neurotransmitter in the rabbit retina .
	manualset3
241331	1	423668	15	NULL	NULL	0	NULL	Arsenic	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Arsenic in soil was examined using Scanning Electron Microscopy coupled with Energy Dispersive X-ray spectroscopy .
	manualset3
241332	2	423668	15	NULL	NULL	0	NULL	soil	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Arsenic in soil was examined using Scanning Electron Microscopy coupled with Energy Dispersive X-ray spectroscopy .
	manualset3
241333	3	423668	15	NULL	NULL	0	NULL	Scanning Electron Microscopy 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Arsenic in soil was examined using Scanning Electron Microscopy coupled with Energy Dispersive X-ray spectroscopy .
	manualset3
241334	4	423668	15	NULL	NULL	0	NULL	Energy Dispersive X-ray spectroscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Arsenic in soil was examined using Scanning Electron Microscopy coupled with Energy Dispersive X-ray spectroscopy .
	manualset3
241335	1	423669	15	NULL	NULL	0	NULL	Arsenic trioxide ( ATO )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Arsenic trioxide ( ATO ) is a first-line anti-cancer agent for acute promyelocytic leukemia , and induces apoptosis in other solid cancer cell lines including breast cancer cells .
	manualset3
241336	2	423669	15	NULL	NULL	0	NULL	first-line anti-cancer agent 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Arsenic trioxide ( ATO ) is a first-line anti-cancer agent for acute promyelocytic leukemia , and induces apoptosis in other solid cancer cell lines including breast cancer cells .
	manualset3
241337	3	423669	15	NULL	NULL	0	NULL	acute promyelocytic leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Arsenic trioxide ( ATO ) is a first-line anti-cancer agent for acute promyelocytic leukemia , and induces apoptosis in other solid cancer cell lines including breast cancer cells .
	manualset3
241338	4	423669	15	NULL	NULL	0	NULL	apoptosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Arsenic trioxide ( ATO ) is a first-line anti-cancer agent for acute promyelocytic leukemia , and induces apoptosis in other solid cancer cell lines including breast cancer cells .
	manualset3
241339	5	423669	15	NULL	NULL	0	NULL	solid cancer cell lines 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Arsenic trioxide ( ATO ) is a first-line anti-cancer agent for acute promyelocytic leukemia , and induces apoptosis in other solid cancer cell lines including breast cancer cells .
	manualset3
241340	6	423669	15	NULL	NULL	0	NULL	breast cancer cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Arsenic trioxide ( ATO ) is a first-line anti-cancer agent for acute promyelocytic leukemia , and induces apoptosis in other solid cancer cell lines including breast cancer cells .
	manualset3
241341	1	423670	15	NULL	NULL	0	NULL	Arterial blood gases analysis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterial blood gases analysis revealed a low PaO2 of 71 mmHg and a decrease of oxygen saturation to 91 % with supplement of fractional oxygen of 35 % .
	manualset3
241342	2	423670	15	NULL	NULL	NULL	NULL	PaO2	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Arterial blood gases analysis revealed a low PaO2 of 71 mmHg and a decrease of oxygen saturation to 91 % with supplement of fractional oxygen of 35 % .
	manualset3
241343	4	423670	15	NULL	NULL	NULL	NULL	decrease	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Arterial blood gases analysis revealed a low PaO2 of 71 mmHg and a decrease of oxygen saturation to 91 % with supplement of fractional oxygen of 35 % .
	manualset3
241344	5	423670	15	NULL	NULL	NULL	NULL	oxygen saturation 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Arterial blood gases analysis revealed a low PaO2 of 71 mmHg and a decrease of oxygen saturation to 91 % with supplement of fractional oxygen of 35 % .
	manualset3
241345	7	423670	15	NULL	NULL	NULL	NULL	supplement 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Arterial blood gases analysis revealed a low PaO2 of 71 mmHg and a decrease of oxygen saturation to 91 % with supplement of fractional oxygen of 35 % .
	manualset3
241346	8	423670	15	NULL	NULL	NULL	NULL	fractional oxygen 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Arterial blood gases analysis revealed a low PaO2 of 71 mmHg and a decrease of oxygen saturation to 91 % with supplement of fractional oxygen of 35 % .
	manualset3
258806	3	423670	15	NULL	NULL	NULL	NULL	71 mmHg	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Arterial blood gases analysis revealed a low PaO2 of 71 mmHg and a decrease of oxygen saturation to 91 % with supplement of fractional oxygen of 35 % .
	manualset3
258809	9	423670	15	NULL	NULL	NULL	NULL	35 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Arterial blood gases analysis revealed a low PaO2 of 71 mmHg and a decrease of oxygen saturation to 91 % with supplement of fractional oxygen of 35 % .
	manualset3
258813	6	423670	15	NULL	NULL	NULL	NULL	91 % 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Arterial blood gases analysis revealed a low PaO2 of 71 mmHg and a decrease of oxygen saturation to 91 % with supplement of fractional oxygen of 35 % .
	manualset3
241347	1	423671	15	NULL	NULL	0	NULL	Effect of internship	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of internship on the Israeli medical graduate ) .
	manualset3
241348	2	423671	15	NULL	NULL	0	NULL	Israeli medical graduate 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of internship on the Israeli medical graduate ) .
	manualset3
241349	1	423672	15	NULL	NULL	0	NULL	Arterial blood pressure	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterial blood pressure , and electrocardiography were continuously monitored for 30min and plasma bupivacaine concentrations at every 5min .
	manualset3
241350	2	423672	15	NULL	NULL	0	NULL	electrocardiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterial blood pressure , and electrocardiography were continuously monitored for 30min and plasma bupivacaine concentrations at every 5min .
	manualset3
241351	3	423672	15	NULL	NULL	0	NULL	30min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterial blood pressure , and electrocardiography were continuously monitored for 30min and plasma bupivacaine concentrations at every 5min .
	manualset3
241352	4	423672	15	NULL	NULL	0	NULL	plasma bupivacaine concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterial blood pressure , and electrocardiography were continuously monitored for 30min and plasma bupivacaine concentrations at every 5min .
	manualset3
241353	5	423672	15	NULL	NULL	NULL	NULL	5min	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Arterial blood pressure , and electrocardiography were continuously monitored for 30min and plasma bupivacaine concentrations at every 5min .
	manualset3
241354	1	423673	15	NULL	NULL	0	NULL	Arterial dissection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterial dissection should be considered in the differential diagnosis of supraclinoid occlusion of the internal carotid artery seen by cerebral angiography .
	manualset3
241355	2	423673	15	NULL	NULL	0	NULL	differential diagnosis of supraclinoid occlusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterial dissection should be considered in the differential diagnosis of supraclinoid occlusion of the internal carotid artery seen by cerebral angiography .
	manualset3
241356	3	423673	15	NULL	NULL	0	NULL	internal carotid artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterial dissection should be considered in the differential diagnosis of supraclinoid occlusion of the internal carotid artery seen by cerebral angiography .
	manualset3
241357	4	423673	15	NULL	NULL	0	NULL	cerebral angiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterial dissection should be considered in the differential diagnosis of supraclinoid occlusion of the internal carotid artery seen by cerebral angiography .
	manualset3
241358	1	423674	15	NULL	NULL	0	NULL	Arterial pressure profile	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterial pressure profile in patients with cirrhosis : Fourier analysis of arterial pulse in relation to pressure level , stroke volume , and severity of disease : On the reduction of afterload in the hyperdynamic syndrome .
	manualset3
241359	2	423674	15	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterial pressure profile in patients with cirrhosis : Fourier analysis of arterial pulse in relation to pressure level , stroke volume , and severity of disease : On the reduction of afterload in the hyperdynamic syndrome .
	manualset3
241360	3	423674	15	NULL	NULL	0	NULL	cirrhosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterial pressure profile in patients with cirrhosis : Fourier analysis of arterial pulse in relation to pressure level , stroke volume , and severity of disease : On the reduction of afterload in the hyperdynamic syndrome .
	manualset3
241361	4	423674	15	NULL	NULL	NULL	NULL	Fourier analysis of arterial pulse	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Arterial pressure profile in patients with cirrhosis : Fourier analysis of arterial pulse in relation to pressure level , stroke volume , and severity of disease : On the reduction of afterload in the hyperdynamic syndrome .
	manualset3
241362	5	423674	15	NULL	NULL	0	NULL	pressure level	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterial pressure profile in patients with cirrhosis : Fourier analysis of arterial pulse in relation to pressure level , stroke volume , and severity of disease : On the reduction of afterload in the hyperdynamic syndrome .
	manualset3
241363	6	423674	15	NULL	NULL	0	NULL	stroke volume	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterial pressure profile in patients with cirrhosis : Fourier analysis of arterial pulse in relation to pressure level , stroke volume , and severity of disease : On the reduction of afterload in the hyperdynamic syndrome .
	manualset3
241364	7	423674	15	NULL	NULL	0	NULL	severity of disease	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterial pressure profile in patients with cirrhosis : Fourier analysis of arterial pulse in relation to pressure level , stroke volume , and severity of disease : On the reduction of afterload in the hyperdynamic syndrome .
	manualset3
241365	8	423674	15	NULL	NULL	0	NULL	reduction of afterload 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterial pressure profile in patients with cirrhosis : Fourier analysis of arterial pulse in relation to pressure level , stroke volume , and severity of disease : On the reduction of afterload in the hyperdynamic syndrome .
	manualset3
241366	9	423674	15	NULL	NULL	0	NULL	hyperdynamic syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Arterial pressure profile in patients with cirrhosis : Fourier analysis of arterial pulse in relation to pressure level , stroke volume , and severity of disease : On the reduction of afterload in the hyperdynamic syndrome .
	manualset3
241367	1	423675	15	NULL	NULL	0	NULL	Arthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Arthritis and tenosynovitis are frequently reported as complications of inflammatory bowel diseases .
	manualset3
241368	2	423675	15	NULL	NULL	0	NULL	tenosynovitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Arthritis and tenosynovitis are frequently reported as complications of inflammatory bowel diseases .
	manualset3
241369	3	423675	15	NULL	NULL	0	NULL	complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Arthritis and tenosynovitis are frequently reported as complications of inflammatory bowel diseases .
	manualset3
241370	4	423675	15	NULL	NULL	0	NULL	inflammatory bowel diseases 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Arthritis and tenosynovitis are frequently reported as complications of inflammatory bowel diseases .
	manualset3
241371	1	423676	15	NULL	NULL	0	NULL	Arthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Arthritis was induced by injecting 0.1 ml of heat killed mycobacterium tuberculosis ( 10 mg/ml of paraffin oil ) intradermally into the left hind paw .
	manualset3
241372	2	423676	15	NULL	NULL	0	NULL	0.1 ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Arthritis was induced by injecting 0.1 ml of heat killed mycobacterium tuberculosis ( 10 mg/ml of paraffin oil ) intradermally into the left hind paw .
	manualset3
241373	3	423676	15	NULL	NULL	0	NULL	heat killed mycobacterium tuberculosis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Arthritis was induced by injecting 0.1 ml of heat killed mycobacterium tuberculosis ( 10 mg/ml of paraffin oil ) intradermally into the left hind paw .
	manualset3
241374	4	423676	15	NULL	NULL	0	NULL	10 mg/ml of paraffin oil	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Arthritis was induced by injecting 0.1 ml of heat killed mycobacterium tuberculosis ( 10 mg/ml of paraffin oil ) intradermally into the left hind paw .
	manualset3
241375	5	423676	15	NULL	NULL	0	NULL	left hind paw	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Arthritis was induced by injecting 0.1 ml of heat killed mycobacterium tuberculosis ( 10 mg/ml of paraffin oil ) intradermally into the left hind paw .
	manualset3
241376	1	423677	15	NULL	NULL	0	NULL	Arthroscopic repair of rotator cuff tear	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Arthroscopic repair of rotator cuff tear with a modified Mason-Allen stitch : mid-term clinical and ultrasound outcomes .
	manualset3
241377	2	423677	15	NULL	NULL	0	NULL	modified Mason-Allen stitch	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Arthroscopic repair of rotator cuff tear with a modified Mason-Allen stitch : mid-term clinical and ultrasound outcomes .
	manualset3
241378	3	423677	15	NULL	NULL	0	NULL	mid-term clinical outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Arthroscopic repair of rotator cuff tear with a modified Mason-Allen stitch : mid-term clinical and ultrasound outcomes .
	manualset3
241379	4	423677	15	NULL	NULL	0	NULL	ultrasound outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Arthroscopic repair of rotator cuff tear with a modified Mason-Allen stitch : mid-term clinical and ultrasound outcomes .
	manualset3
241380	1	423678	15	NULL	NULL	0	NULL	CPT I kinetics	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As CPT I kinetics are highly dependent on its membrane environment , we have measured the kinetic parameters of CPT I present in rat liver submitochondrial membrane fractions enriched in either outer membrane or contact sites .
	manualset3
241381	2	423678	15	NULL	NULL	0	NULL	membrane environment 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As CPT I kinetics are highly dependent on its membrane environment , we have measured the kinetic parameters of CPT I present in rat liver submitochondrial membrane fractions enriched in either outer membrane or contact sites .
	manualset3
241382	3	423678	15	NULL	NULL	0	NULL	kinetic parameters of CPT I	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As CPT I kinetics are highly dependent on its membrane environment , we have measured the kinetic parameters of CPT I present in rat liver submitochondrial membrane fractions enriched in either outer membrane or contact sites .
	manualset3
241383	4	423678	15	NULL	NULL	0	NULL	rat liver submitochondrial membrane fractions	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	As CPT I kinetics are highly dependent on its membrane environment , we have measured the kinetic parameters of CPT I present in rat liver submitochondrial membrane fractions enriched in either outer membrane or contact sites .
	manualset3
241384	5	423678	15	NULL	NULL	0	NULL	outer membrane	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	As CPT I kinetics are highly dependent on its membrane environment , we have measured the kinetic parameters of CPT I present in rat liver submitochondrial membrane fractions enriched in either outer membrane or contact sites .
	manualset3
241385	6	423678	15	NULL	NULL	0	NULL	contact sites	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	As CPT I kinetics are highly dependent on its membrane environment , we have measured the kinetic parameters of CPT I present in rat liver submitochondrial membrane fractions enriched in either outer membrane or contact sites .
	manualset3
241386	1	423679	15	NULL	NULL	0	NULL	case	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( A case of successful plastic repair of a defect of the orbital wall with preserved homologous cartilage ) .
	manualset3
241387	2	423679	15	NULL	NULL	0	NULL	plastic repair 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( A case of successful plastic repair of a defect of the orbital wall with preserved homologous cartilage ) .
	manualset3
241388	3	423679	15	NULL	NULL	0	NULL	defect of the orbital wall	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( A case of successful plastic repair of a defect of the orbital wall with preserved homologous cartilage ) .
	manualset3
241389	4	423679	15	NULL	NULL	0	NULL	homologous cartilage	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	( A case of successful plastic repair of a defect of the orbital wall with preserved homologous cartilage ) .
	manualset3
241390	1	423680	15	NULL	NULL	0	NULL	combination therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As a combination therapy , mice in the other group were treated with intra-tumoral injection of adenoviral vector carrying IL-18 gene ( Ad.IL-18 ) .
	manualset3
241391	2	423680	15	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	As a combination therapy , mice in the other group were treated with intra-tumoral injection of adenoviral vector carrying IL-18 gene ( Ad.IL-18 ) .
	manualset3
241392	3	423680	15	NULL	NULL	0	NULL	group 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	As a combination therapy , mice in the other group were treated with intra-tumoral injection of adenoviral vector carrying IL-18 gene ( Ad.IL-18 ) .
	manualset3
241393	4	423680	15	NULL	NULL	0	NULL	intra-tumoral injection 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	As a combination therapy , mice in the other group were treated with intra-tumoral injection of adenoviral vector carrying IL-18 gene ( Ad.IL-18 ) .
	manualset3
241394	5	423680	15	NULL	NULL	0	NULL	adenoviral vector carrying IL-18 gene ( Ad.IL-18 )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	As a combination therapy , mice in the other group were treated with intra-tumoral injection of adenoviral vector carrying IL-18 gene ( Ad.IL-18 ) .
	manualset3
241395	1	423681	15	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	As a comparison , we also formed the network structure on mica substrate .
	manualset3
241396	2	423681	15	NULL	NULL	0	NULL	network structure 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As a comparison , we also formed the network structure on mica substrate .
	manualset3
241397	3	423681	15	NULL	NULL	NULL	NULL	mica substrate 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As a comparison , we also formed the network structure on mica substrate .
	manualset3
241398	1	423682	15	NULL	NULL	0	NULL	consequence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As a consequence , defects of the membrane structure are developed to assist permeation .
	manualset3
241399	2	423682	15	NULL	NULL	0	NULL	defects of the membrane structure 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As a consequence , defects of the membrane structure are developed to assist permeation .
	manualset3
241400	3	423682	15	NULL	NULL	0	NULL	permeation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As a consequence , defects of the membrane structure are developed to assist permeation .
	manualset3
241401	1	423683	15	NULL	NULL	0	NULL	consequence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As a consequence , hydrophobic moment plot methodology is often used to identify putative transmembrane alpha-helices of integral membrane proteins , based on their local maximum mean hydrophobic moment ( & lt ; microH ) ) and the corresponding mean hydrophobicity ( & lt ; H ) ) .
	manualset3
241402	2	423683	15	NULL	NULL	0	NULL	hydrophobic moment plot methodology	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	As a consequence , hydrophobic moment plot methodology is often used to identify putative transmembrane alpha-helices of integral membrane proteins , based on their local maximum mean hydrophobic moment ( & lt ; microH ) ) and the corresponding mean hydrophobicity ( & lt ; H ) ) .
	manualset3
241403	3	423683	15	NULL	NULL	0	NULL	putative transmembrane alpha-helices	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As a consequence , hydrophobic moment plot methodology is often used to identify putative transmembrane alpha-helices of integral membrane proteins , based on their local maximum mean hydrophobic moment ( & lt ; microH ) ) and the corresponding mean hydrophobicity ( & lt ; H ) ) .
	manualset3
241404	4	423683	15	NULL	NULL	0	NULL	integral membrane proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As a consequence , hydrophobic moment plot methodology is often used to identify putative transmembrane alpha-helices of integral membrane proteins , based on their local maximum mean hydrophobic moment ( & lt ; microH ) ) and the corresponding mean hydrophobicity ( & lt ; H ) ) .
	manualset3
241405	5	423683	15	NULL	NULL	0	NULL	local maximum mean hydrophobic moment ( & lt ; microH )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As a consequence , hydrophobic moment plot methodology is often used to identify putative transmembrane alpha-helices of integral membrane proteins , based on their local maximum mean hydrophobic moment ( & lt ; microH ) ) and the corresponding mean hydrophobicity ( & lt ; H ) ) .
	manualset3
241406	6	423683	15	NULL	NULL	0	NULL	corresponding mean hydrophobicity ( & lt ; H ) 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As a consequence , hydrophobic moment plot methodology is often used to identify putative transmembrane alpha-helices of integral membrane proteins , based on their local maximum mean hydrophobic moment ( & lt ; microH ) ) and the corresponding mean hydrophobicity ( & lt ; H ) ) .
	manualset3
241407	1	423684	15	NULL	NULL	0	NULL	consequence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As a consequence , more than 16 % of individuals were misclassified in terms of the NCEP risk category into which their Reflotron readings fell .
	manualset3
241408	2	423684	15	NULL	NULL	0	NULL	16 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As a consequence , more than 16 % of individuals were misclassified in terms of the NCEP risk category into which their Reflotron readings fell .
	manualset3
241409	3	423684	15	NULL	NULL	0	NULL	individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As a consequence , more than 16 % of individuals were misclassified in terms of the NCEP risk category into which their Reflotron readings fell .
	manualset3
241410	4	423684	15	NULL	NULL	0	NULL	NCEP risk category	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As a consequence , more than 16 % of individuals were misclassified in terms of the NCEP risk category into which their Reflotron readings fell .
	manualset3
241411	5	423684	15	NULL	NULL	0	NULL	Reflotron readings	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As a consequence , more than 16 % of individuals were misclassified in terms of the NCEP risk category into which their Reflotron readings fell .
	manualset3
241412	1	423685	15	NULL	NULL	0	NULL	consequence of the illness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As a consequence of the illness , the relationship between caregiver and care recipient frequently becomes closer and deeper , although it is important that they both maintain hope for the future .
	manualset3
241413	2	423685	15	NULL	NULL	0	NULL	relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	As a consequence of the illness , the relationship between caregiver and care recipient frequently becomes closer and deeper , although it is important that they both maintain hope for the future .
	manualset3
241414	3	423685	15	NULL	NULL	0	NULL	caregiver	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	As a consequence of the illness , the relationship between caregiver and care recipient frequently becomes closer and deeper , although it is important that they both maintain hope for the future .
	manualset3
241415	4	423685	15	NULL	NULL	0	NULL	care recipient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	As a consequence of the illness , the relationship between caregiver and care recipient frequently becomes closer and deeper , although it is important that they both maintain hope for the future .
	manualset3
241416	5	423685	15	NULL	NULL	0	NULL	hope	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As a consequence of the illness , the relationship between caregiver and care recipient frequently becomes closer and deeper , although it is important that they both maintain hope for the future .
	manualset3
241417	6	423685	15	NULL	NULL	0	NULL	future	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	As a consequence of the illness , the relationship between caregiver and care recipient frequently becomes closer and deeper , although it is important that they both maintain hope for the future .
	manualset3
241419	1	423686	15	NULL	NULL	NULL	NULL	step	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As a first step in developing a molecular method for the individualization of marijuana samples , we evaluated a plant DNA extraction kit .
	manualset3
241422	2	423686	15	NULL	NULL	NULL	NULL	developing a molecular method 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As a first step in developing a molecular method for the individualization of marijuana samples , we evaluated a plant DNA extraction kit .
	manualset3
241424	3	423686	15	NULL	NULL	0	NULL	individualization of marijuana samples	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	As a first step in developing a molecular method for the individualization of marijuana samples , we evaluated a plant DNA extraction kit .
	manualset3
241425	4	423686	15	NULL	NULL	0	NULL	plant DNA extraction kit	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	As a first step in developing a molecular method for the individualization of marijuana samples , we evaluated a plant DNA extraction kit .
	manualset3
241426	1	423687	15	NULL	NULL	NULL	NULL	general clinical guide	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As a general clinical guide , each degree of rotation of the occlusal plane will result in a half millimeter change in the dental occlusal relationship .
	manualset3
241428	2	423687	15	NULL	NULL	0	NULL	each degree of rotation of the occlusal plane	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As a general clinical guide , each degree of rotation of the occlusal plane will result in a half millimeter change in the dental occlusal relationship .
	manualset3
241431	3	423687	15	NULL	NULL	0	NULL	half millimeter change 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As a general clinical guide , each degree of rotation of the occlusal plane will result in a half millimeter change in the dental occlusal relationship .
	manualset3
241432	4	423687	15	NULL	NULL	0	NULL	dental occlusal relationship 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	As a general clinical guide , each degree of rotation of the occlusal plane will result in a half millimeter change in the dental occlusal relationship .
	manualset3
241433	1	423688	15	NULL	NULL	0	NULL	general rule	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	As a general rule , however , older cardiac transplant patients should be treated with lower doses and fewer immunosuppressive drugs to avoid over-immunosuppression .
	manualset3
241434	2	423688	15	NULL	NULL	0	NULL	older cardiac transplant patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As a general rule , however , older cardiac transplant patients should be treated with lower doses and fewer immunosuppressive drugs to avoid over-immunosuppression .
	manualset3
241435	3	423688	15	NULL	NULL	0	NULL	doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	As a general rule , however , older cardiac transplant patients should be treated with lower doses and fewer immunosuppressive drugs to avoid over-immunosuppression .
	manualset3
241436	4	423688	15	NULL	NULL	0	NULL	immunosuppressive drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	As a general rule , however , older cardiac transplant patients should be treated with lower doses and fewer immunosuppressive drugs to avoid over-immunosuppression .
	manualset3
241437	5	423688	15	NULL	NULL	0	NULL	over-immunosuppression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As a general rule , however , older cardiac transplant patients should be treated with lower doses and fewer immunosuppressive drugs to avoid over-immunosuppression .
	manualset3
241438	1	423689	15	NULL	NULL	0	NULL	Effect of sera 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of sera from children with acute lymphoblastic leukemia on the morphology of granulocyte-macrophage colonies grown from murine bone marrow cells and the cells of murine myelomonocytic leukemia WEHI 3B D + ) .
	manualset3
241439	2	423689	15	NULL	NULL	0	NULL	children 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of sera from children with acute lymphoblastic leukemia on the morphology of granulocyte-macrophage colonies grown from murine bone marrow cells and the cells of murine myelomonocytic leukemia WEHI 3B D + ) .
	manualset3
241441	3	423689	15	NULL	NULL	0	NULL	acute lymphoblastic leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of sera from children with acute lymphoblastic leukemia on the morphology of granulocyte-macrophage colonies grown from murine bone marrow cells and the cells of murine myelomonocytic leukemia WEHI 3B D + ) .
	manualset3
241443	4	423689	15	NULL	NULL	0	NULL	morphology of granulocyte-macrophage colonies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of sera from children with acute lymphoblastic leukemia on the morphology of granulocyte-macrophage colonies grown from murine bone marrow cells and the cells of murine myelomonocytic leukemia WEHI 3B D + ) .
	manualset3
241445	5	423689	15	NULL	NULL	0	NULL	murine bone marrow cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of sera from children with acute lymphoblastic leukemia on the morphology of granulocyte-macrophage colonies grown from murine bone marrow cells and the cells of murine myelomonocytic leukemia WEHI 3B D + ) .
	manualset3
241446	6	423689	15	NULL	NULL	0	NULL	cells of murine myelomonocytic leukemia WEHI 3B D +	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of sera from children with acute lymphoblastic leukemia on the morphology of granulocyte-macrophage colonies grown from murine bone marrow cells and the cells of murine myelomonocytic leukemia WEHI 3B D + ) .
	manualset3
241449	1	423690	15	NULL	NULL	0	NULL	group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As a group and individually , patients had significantly higher levels of serum total calcium , ionized calcium , and parathyroid hormone .
	manualset3
241450	2	423690	15	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As a group and individually , patients had significantly higher levels of serum total calcium , ionized calcium , and parathyroid hormone .
	manualset3
241451	3	423690	15	NULL	NULL	0	NULL	levels of serum total calcium	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As a group and individually , patients had significantly higher levels of serum total calcium , ionized calcium , and parathyroid hormone .
	manualset3
241452	4	423690	15	NULL	NULL	0	NULL	levels of ionized calcium	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As a group and individually , patients had significantly higher levels of serum total calcium , ionized calcium , and parathyroid hormone .
	manualset3
241453	5	423690	15	NULL	NULL	0	NULL	levels of parathyroid hormone	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As a group and individually , patients had significantly higher levels of serum total calcium , ionized calcium , and parathyroid hormone .
	manualset3
241455	1	423691	15	NULL	NULL	0	NULL	octreotide 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	As a matter of fact , the octreotide coadministered with caerulein counteracted the caerulein-induced increase of pancreatic DNA content and therefore acted against the reactive pancreatic hyperplasia .
	manualset3
241458	2	423691	15	NULL	NULL	0	NULL	caerulein 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	As a matter of fact , the octreotide coadministered with caerulein counteracted the caerulein-induced increase of pancreatic DNA content and therefore acted against the reactive pancreatic hyperplasia .
	manualset3
241460	3	423691	15	NULL	NULL	0	NULL	caerulein-induced increase of pancreatic DNA content 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As a matter of fact , the octreotide coadministered with caerulein counteracted the caerulein-induced increase of pancreatic DNA content and therefore acted against the reactive pancreatic hyperplasia .
	manualset3
241461	4	423691	15	NULL	NULL	0	NULL	reactive pancreatic hyperplasia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	As a matter of fact , the octreotide coadministered with caerulein counteracted the caerulein-induced increase of pancreatic DNA content and therefore acted against the reactive pancreatic hyperplasia .
	manualset3
241463	1	423692	15	NULL	NULL	0	NULL	model compound	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	As a model compound , well-characterized nanospheres imprinted against L : - Boc-phenylalanine anilide ( L : - BFA ) were chosen .
	manualset3
241471	2	423692	15	NULL	NULL	0	NULL	nanospheres	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	As a model compound , well-characterized nanospheres imprinted against L : - Boc-phenylalanine anilide ( L : - BFA ) were chosen .
	manualset3
241479	3	423692	15	NULL	NULL	0	NULL	L : - Boc-phenylalanine anilide ( L : - BFA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	As a model compound , well-characterized nanospheres imprinted against L : - Boc-phenylalanine anilide ( L : - BFA ) were chosen .
	manualset3
241480	1	423693	15	NULL	NULL	0	NULL	part	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As a part of a comprehensive therapy monitoring 65 patients with therapy refractory epilepsy were studied with the Freiburg Questionnaire of coping with Illness ( FKV ) on the day after admittance to a specialized epilepsy ward .
	manualset3
241481	2	423693	15	NULL	NULL	0	NULL	comprehensive therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As a part of a comprehensive therapy monitoring 65 patients with therapy refractory epilepsy were studied with the Freiburg Questionnaire of coping with Illness ( FKV ) on the day after admittance to a specialized epilepsy ward .
	manualset3
241482	3	423693	15	NULL	NULL	0	NULL	65 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As a part of a comprehensive therapy monitoring 65 patients with therapy refractory epilepsy were studied with the Freiburg Questionnaire of coping with Illness ( FKV ) on the day after admittance to a specialized epilepsy ward .
	manualset3
241483	4	423693	15	NULL	NULL	0	NULL	therapy refractory epilepsy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As a part of a comprehensive therapy monitoring 65 patients with therapy refractory epilepsy were studied with the Freiburg Questionnaire of coping with Illness ( FKV ) on the day after admittance to a specialized epilepsy ward .
	manualset3
241484	5	423693	15	NULL	NULL	0	NULL	Freiburg Questionnaire 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	As a part of a comprehensive therapy monitoring 65 patients with therapy refractory epilepsy were studied with the Freiburg Questionnaire of coping with Illness ( FKV ) on the day after admittance to a specialized epilepsy ward .
	manualset3
241485	6	423693	15	NULL	NULL	0	NULL	Illness ( FKV ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As a part of a comprehensive therapy monitoring 65 patients with therapy refractory epilepsy were studied with the Freiburg Questionnaire of coping with Illness ( FKV ) on the day after admittance to a specialized epilepsy ward .
	manualset3
241486	7	423693	15	NULL	NULL	NULL	NULL	day after admittance	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As a part of a comprehensive therapy monitoring 65 patients with therapy refractory epilepsy were studied with the Freiburg Questionnaire of coping with Illness ( FKV ) on the day after admittance to a specialized epilepsy ward .
	manualset3
241487	8	423693	15	NULL	NULL	0	NULL	specialized epilepsy ward 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	As a part of a comprehensive therapy monitoring 65 patients with therapy refractory epilepsy were studied with the Freiburg Questionnaire of coping with Illness ( FKV ) on the day after admittance to a specialized epilepsy ward .
	manualset3
241488	1	423694	15	NULL	NULL	0	NULL	positive control	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	As a positive control , ghrelin showed saturable binding and endocytosis in RBE4 cerebral microvessel endothelial cells .
	manualset3
241489	2	423694	15	NULL	NULL	0	NULL	ghrelin	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	As a positive control , ghrelin showed saturable binding and endocytosis in RBE4 cerebral microvessel endothelial cells .
	manualset3
241490	3	423694	15	NULL	NULL	0	NULL	saturable binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As a positive control , ghrelin showed saturable binding and endocytosis in RBE4 cerebral microvessel endothelial cells .
	manualset3
241491	4	423694	15	NULL	NULL	0	NULL	endocytosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As a positive control , ghrelin showed saturable binding and endocytosis in RBE4 cerebral microvessel endothelial cells .
	manualset3
241492	5	423694	15	NULL	NULL	0	NULL	RBE4 cerebral microvessel endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	As a positive control , ghrelin showed saturable binding and endocytosis in RBE4 cerebral microvessel endothelial cells .
	manualset3
241493	1	423695	15	NULL	NULL	0	NULL	potential screening test 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	As a potential screening test with a 5-year interval for men under 65 , the sensitivity would be 92 % and specificity 97 % .
	manualset3
241494	2	423695	15	NULL	NULL	0	NULL	5-year interval 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	As a potential screening test with a 5-year interval for men under 65 , the sensitivity would be 92 % and specificity 97 % .
	manualset3
241495	3	423695	15	NULL	NULL	NULL	NULL	men under 65 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As a potential screening test with a 5-year interval for men under 65 , the sensitivity would be 92 % and specificity 97 % .
	manualset3
241496	4	423695	15	NULL	NULL	0	NULL	sensitivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As a potential screening test with a 5-year interval for men under 65 , the sensitivity would be 92 % and specificity 97 % .
	manualset3
241497	5	423695	15	NULL	NULL	0	NULL	92 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As a potential screening test with a 5-year interval for men under 65 , the sensitivity would be 92 % and specificity 97 % .
	manualset3
241498	6	423695	15	NULL	NULL	0	NULL	specificity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As a potential screening test with a 5-year interval for men under 65 , the sensitivity would be 92 % and specificity 97 % .
	manualset3
241499	7	423695	15	NULL	NULL	0	NULL	97 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As a potential screening test with a 5-year interval for men under 65 , the sensitivity would be 92 % and specificity 97 % .
	manualset3
241500	1	423696	15	NULL	NULL	0	NULL	predictive test 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As a predictive test , plasma TDP-43 level may have great practical value in directing therapeutic strategies aimed at preventing or removing tau or TDP-43 pathological changes from the brain in FTLD and AD .
	manualset3
241501	2	423696	15	NULL	NULL	0	NULL	plasma TDP-43 level	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As a predictive test , plasma TDP-43 level may have great practical value in directing therapeutic strategies aimed at preventing or removing tau or TDP-43 pathological changes from the brain in FTLD and AD .
	manualset3
241502	3	423696	15	NULL	NULL	0	NULL	practical value	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As a predictive test , plasma TDP-43 level may have great practical value in directing therapeutic strategies aimed at preventing or removing tau or TDP-43 pathological changes from the brain in FTLD and AD .
	manualset3
241503	4	423696	15	NULL	NULL	0	NULL	therapeutic strategies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As a predictive test , plasma TDP-43 level may have great practical value in directing therapeutic strategies aimed at preventing or removing tau or TDP-43 pathological changes from the brain in FTLD and AD .
	manualset3
241504	5	423696	15	NULL	NULL	0	NULL	tau or TDP-43 pathological changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As a predictive test , plasma TDP-43 level may have great practical value in directing therapeutic strategies aimed at preventing or removing tau or TDP-43 pathological changes from the brain in FTLD and AD .
	manualset3
241505	6	423696	15	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	As a predictive test , plasma TDP-43 level may have great practical value in directing therapeutic strategies aimed at preventing or removing tau or TDP-43 pathological changes from the brain in FTLD and AD .
	manualset3
241506	7	423696	15	NULL	NULL	0	NULL	FTLD	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As a predictive test , plasma TDP-43 level may have great practical value in directing therapeutic strategies aimed at preventing or removing tau or TDP-43 pathological changes from the brain in FTLD and AD .
	manualset3
241507	8	423696	15	NULL	NULL	0	NULL	AD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	As a predictive test , plasma TDP-43 level may have great practical value in directing therapeutic strategies aimed at preventing or removing tau or TDP-43 pathological changes from the brain in FTLD and AD .
	manualset3
241508	1	423697	15	NULL	NULL	0	NULL	result	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result , the more mature stages of Plasmodium falciparum are sequestered in the microvasculature and cause vital organ dysfunction , whereas the ring stages circulate in the blood stream .
	manualset3
241509	2	423697	15	NULL	NULL	0	NULL	mature stages of Plasmodium falciparum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result , the more mature stages of Plasmodium falciparum are sequestered in the microvasculature and cause vital organ dysfunction , whereas the ring stages circulate in the blood stream .
	manualset3
241510	3	423697	15	NULL	NULL	0	NULL	microvasculature	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result , the more mature stages of Plasmodium falciparum are sequestered in the microvasculature and cause vital organ dysfunction , whereas the ring stages circulate in the blood stream .
	manualset3
241511	4	423697	15	NULL	NULL	0	NULL	vital organ dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result , the more mature stages of Plasmodium falciparum are sequestered in the microvasculature and cause vital organ dysfunction , whereas the ring stages circulate in the blood stream .
	manualset3
241512	5	423697	15	NULL	NULL	0	NULL	ring stages	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result , the more mature stages of Plasmodium falciparum are sequestered in the microvasculature and cause vital organ dysfunction , whereas the ring stages circulate in the blood stream .
	manualset3
241513	6	423697	15	NULL	NULL	0	NULL	blood stream	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result , the more mature stages of Plasmodium falciparum are sequestered in the microvasculature and cause vital organ dysfunction , whereas the ring stages circulate in the blood stream .
	manualset3
241514	1	423698	15	NULL	NULL	0	NULL	Effect of siRNA transfection	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of siRNA transfection targeting VEGF gene on proliferation and apoptosis of human breast cancer cells ) .
	manualset3
241515	2	423698	15	NULL	NULL	0	NULL	VEGF gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of siRNA transfection targeting VEGF gene on proliferation and apoptosis of human breast cancer cells ) .
	manualset3
241516	3	423698	15	NULL	NULL	0	NULL	proliferation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of siRNA transfection targeting VEGF gene on proliferation and apoptosis of human breast cancer cells ) .
	manualset3
241517	4	423698	15	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of siRNA transfection targeting VEGF gene on proliferation and apoptosis of human breast cancer cells ) .
	manualset3
241518	5	423698	15	NULL	NULL	0	NULL	human breast cancer cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effect of siRNA transfection targeting VEGF gene on proliferation and apoptosis of human breast cancer cells ) .
	manualset3
241519	1	423699	15	NULL	NULL	0	NULL	Legionella pneumophila serogroup 4	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result , we successfully isolated Legionella pneumophila serogroup 4 from hot spring water ( 42 degrees C ) from the bath .
	manualset3
241520	2	423699	15	NULL	NULL	0	NULL	hot spring water	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result , we successfully isolated Legionella pneumophila serogroup 4 from hot spring water ( 42 degrees C ) from the bath .
	manualset3
241521	3	423699	15	NULL	NULL	0	NULL	42 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result , we successfully isolated Legionella pneumophila serogroup 4 from hot spring water ( 42 degrees C ) from the bath .
	manualset3
241522	4	423699	15	NULL	NULL	0	NULL	bath	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result , we successfully isolated Legionella pneumophila serogroup 4 from hot spring water ( 42 degrees C ) from the bath .
	manualset3
241523	1	423700	15	NULL	NULL	NULL	NULL	long term discontinuous stimulation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As a result of long term discontinuous stimulation , secondary changes occur at sites downstream from the dopamine system and now appear to underlie the progressive worsening of ` wearing-off ' phenomena as well as the eventual appearance of other response complications .
	manualset3
241524	2	423700	15	NULL	NULL	0	NULL	secondary changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result of long term discontinuous stimulation , secondary changes occur at sites downstream from the dopamine system and now appear to underlie the progressive worsening of ` wearing-off ' phenomena as well as the eventual appearance of other response complications .
	manualset3
241525	3	423700	15	NULL	NULL	0	NULL	sites downstream from the dopamine system	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result of long term discontinuous stimulation , secondary changes occur at sites downstream from the dopamine system and now appear to underlie the progressive worsening of ` wearing-off ' phenomena as well as the eventual appearance of other response complications .
	manualset3
241526	4	423700	15	NULL	NULL	NULL	NULL	progressive worsening of ` wearing-off ' phenomena 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As a result of long term discontinuous stimulation , secondary changes occur at sites downstream from the dopamine system and now appear to underlie the progressive worsening of ` wearing-off ' phenomena as well as the eventual appearance of other response complications .
	manualset3
241527	5	423700	15	NULL	NULL	0	NULL	eventual appearance 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result of long term discontinuous stimulation , secondary changes occur at sites downstream from the dopamine system and now appear to underlie the progressive worsening of ` wearing-off ' phenomena as well as the eventual appearance of other response complications .
	manualset3
241528	6	423700	15	NULL	NULL	0	NULL	response complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result of long term discontinuous stimulation , secondary changes occur at sites downstream from the dopamine system and now appear to underlie the progressive worsening of ` wearing-off ' phenomena as well as the eventual appearance of other response complications .
	manualset3
241529	1	423701	15	NULL	NULL	0	NULL	proliferation of prostate cancer-specific survey instruments	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result of the proliferation of prostate cancer-specific survey instruments and inconsistencies in their design and application , decision-makers face great difficulties evaluating HR-QOL across disease stages and comparing the HR-QOL impacts of alternative therapies , including conservative management ( ` watchful waiting ' ) .
	manualset3
241530	2	423701	15	NULL	NULL	NULL	NULL	inconsistencies in their design	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As a result of the proliferation of prostate cancer-specific survey instruments and inconsistencies in their design and application , decision-makers face great difficulties evaluating HR-QOL across disease stages and comparing the HR-QOL impacts of alternative therapies , including conservative management ( ` watchful waiting ' ) .
	manualset3
241531	3	423701	15	NULL	NULL	0	NULL	inconsistencies in their application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result of the proliferation of prostate cancer-specific survey instruments and inconsistencies in their design and application , decision-makers face great difficulties evaluating HR-QOL across disease stages and comparing the HR-QOL impacts of alternative therapies , including conservative management ( ` watchful waiting ' ) .
	manualset3
241532	4	423701	15	NULL	NULL	0	NULL	decision-makers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result of the proliferation of prostate cancer-specific survey instruments and inconsistencies in their design and application , decision-makers face great difficulties evaluating HR-QOL across disease stages and comparing the HR-QOL impacts of alternative therapies , including conservative management ( ` watchful waiting ' ) .
	manualset3
241533	5	423701	15	NULL	NULL	0	NULL	difficulties	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result of the proliferation of prostate cancer-specific survey instruments and inconsistencies in their design and application , decision-makers face great difficulties evaluating HR-QOL across disease stages and comparing the HR-QOL impacts of alternative therapies , including conservative management ( ` watchful waiting ' ) .
	manualset3
241534	6	423701	15	NULL	NULL	0	NULL	evaluating HR-QOL across disease stages	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result of the proliferation of prostate cancer-specific survey instruments and inconsistencies in their design and application , decision-makers face great difficulties evaluating HR-QOL across disease stages and comparing the HR-QOL impacts of alternative therapies , including conservative management ( ` watchful waiting ' ) .
	manualset3
241535	7	423701	15	NULL	NULL	0	NULL	comparing the HR-QOL impacts 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result of the proliferation of prostate cancer-specific survey instruments and inconsistencies in their design and application , decision-makers face great difficulties evaluating HR-QOL across disease stages and comparing the HR-QOL impacts of alternative therapies , including conservative management ( ` watchful waiting ' ) .
	manualset3
241536	8	423701	15	NULL	NULL	0	NULL	alternative therapies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result of the proliferation of prostate cancer-specific survey instruments and inconsistencies in their design and application , decision-makers face great difficulties evaluating HR-QOL across disease stages and comparing the HR-QOL impacts of alternative therapies , including conservative management ( ` watchful waiting ' ) .
	manualset3
241537	9	423701	15	NULL	NULL	0	NULL	conservative management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result of the proliferation of prostate cancer-specific survey instruments and inconsistencies in their design and application , decision-makers face great difficulties evaluating HR-QOL across disease stages and comparing the HR-QOL impacts of alternative therapies , including conservative management ( ` watchful waiting ' ) .
	manualset3
241538	10	423701	15	NULL	NULL	0	NULL	watchful waiting	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result of the proliferation of prostate cancer-specific survey instruments and inconsistencies in their design and application , decision-makers face great difficulties evaluating HR-QOL across disease stages and comparing the HR-QOL impacts of alternative therapies , including conservative management ( ` watchful waiting ' ) .
	manualset3
241539	1	423702	15	NULL	NULL	0	NULL	ongoing advances in the prenatal detection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result of these ongoing advances in the prenatal detection and assessment of congenital heart disease , these are exciting and glorious times for the field of fetal cardiac imaging .
	manualset3
241540	2	423702	15	NULL	NULL	0	NULL	assessment of congenital heart disease	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result of these ongoing advances in the prenatal detection and assessment of congenital heart disease , these are exciting and glorious times for the field of fetal cardiac imaging .
	manualset3
241541	3	423702	15	NULL	NULL	0	NULL	times	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result of these ongoing advances in the prenatal detection and assessment of congenital heart disease , these are exciting and glorious times for the field of fetal cardiac imaging .
	manualset3
241542	4	423702	15	NULL	NULL	0	NULL	 field of fetal cardiac imaging	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	As a result of these ongoing advances in the prenatal detection and assessment of congenital heart disease , these are exciting and glorious times for the field of fetal cardiac imaging .
	manualset3
241543	1	423703	15	NULL	NULL	0	NULL	experimental variable	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	As a third experimental variable , lipopolysaccharide was added to the medium .
	manualset3
241544	2	423703	15	NULL	NULL	0	NULL	lipopolysaccharide 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	As a third experimental variable , lipopolysaccharide was added to the medium .
	manualset3
241545	3	423703	15	NULL	NULL	0	NULL	medium 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	As a third experimental variable , lipopolysaccharide was added to the medium .
	manualset3
241546	1	423704	15	NULL	NULL	NULL	NULL	apprarent markers	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As apprarent markers for increased cancer risk , atypical lobules in the human breast may be homologous to hyperplastic alveolar nodules that are abundant in high mammary cancer strains of mice .
	manualset3
241547	2	423704	15	NULL	NULL	0	NULL	increased cancer risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As apprarent markers for increased cancer risk , atypical lobules in the human breast may be homologous to hyperplastic alveolar nodules that are abundant in high mammary cancer strains of mice .
	manualset3
241548	3	423704	15	NULL	NULL	0	NULL	atypical lobules	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As apprarent markers for increased cancer risk , atypical lobules in the human breast may be homologous to hyperplastic alveolar nodules that are abundant in high mammary cancer strains of mice .
	manualset3
241549	4	423704	15	NULL	NULL	0	NULL	human breast	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	As apprarent markers for increased cancer risk , atypical lobules in the human breast may be homologous to hyperplastic alveolar nodules that are abundant in high mammary cancer strains of mice .
	manualset3
241550	5	423704	15	NULL	NULL	0	NULL	homologous	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	As apprarent markers for increased cancer risk , atypical lobules in the human breast may be homologous to hyperplastic alveolar nodules that are abundant in high mammary cancer strains of mice .
	manualset3
241551	6	423704	15	NULL	NULL	0	NULL	hyperplastic alveolar nodules 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As apprarent markers for increased cancer risk , atypical lobules in the human breast may be homologous to hyperplastic alveolar nodules that are abundant in high mammary cancer strains of mice .
	manualset3
241552	7	423704	15	NULL	NULL	0	NULL	mammary cancer strains of mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	As apprarent markers for increased cancer risk , atypical lobules in the human breast may be homologous to hyperplastic alveolar nodules that are abundant in high mammary cancer strains of mice .
	manualset3
241553	1	423705	15	NULL	NULL	0	NULL	astrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	As astrocytes are known to secrete immunomodulatory and neuroprotective substances , we investigated whether astrocytic factors can attenuate the amount of neuronal injury as well as the degree of microglial activation in a model of excitotoxic neurodegeneration .
	manualset3
241554	2	423705	15	NULL	NULL	0	NULL	immunomodulatory substances	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As astrocytes are known to secrete immunomodulatory and neuroprotective substances , we investigated whether astrocytic factors can attenuate the amount of neuronal injury as well as the degree of microglial activation in a model of excitotoxic neurodegeneration .
	manualset3
241555	3	423705	15	NULL	NULL	0	NULL	neuroprotective substances 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As astrocytes are known to secrete immunomodulatory and neuroprotective substances , we investigated whether astrocytic factors can attenuate the amount of neuronal injury as well as the degree of microglial activation in a model of excitotoxic neurodegeneration .
	manualset3
241556	4	423705	15	NULL	NULL	0	NULL	astrocytic factors 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As astrocytes are known to secrete immunomodulatory and neuroprotective substances , we investigated whether astrocytic factors can attenuate the amount of neuronal injury as well as the degree of microglial activation in a model of excitotoxic neurodegeneration .
	manualset3
241557	5	423705	15	NULL	NULL	0	NULL	amount of neuronal injury 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As astrocytes are known to secrete immunomodulatory and neuroprotective substances , we investigated whether astrocytic factors can attenuate the amount of neuronal injury as well as the degree of microglial activation in a model of excitotoxic neurodegeneration .
	manualset3
241558	6	423705	15	NULL	NULL	0	NULL	degree of microglial activation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As astrocytes are known to secrete immunomodulatory and neuroprotective substances , we investigated whether astrocytic factors can attenuate the amount of neuronal injury as well as the degree of microglial activation in a model of excitotoxic neurodegeneration .
	manualset3
241559	7	423705	15	NULL	NULL	0	NULL	model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	As astrocytes are known to secrete immunomodulatory and neuroprotective substances , we investigated whether astrocytic factors can attenuate the amount of neuronal injury as well as the degree of microglial activation in a model of excitotoxic neurodegeneration .
	manualset3
241560	8	423705	15	NULL	NULL	0	NULL	excitotoxic neurodegeneration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As astrocytes are known to secrete immunomodulatory and neuroprotective substances , we investigated whether astrocytic factors can attenuate the amount of neuronal injury as well as the degree of microglial activation in a model of excitotoxic neurodegeneration .
	manualset3
241561	1	423706	15	NULL	NULL	0	NULL	bovine spongiform encephalopathy ( BSE ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	As bovine spongiform encephalopathy ( BSE ) has not been reported in Austria , the data do not support a link between a rise in incidence of sporadic CJD and BSE .
	manualset3
241562	2	423706	15	NULL	NULL	0	NULL	Austria	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	As bovine spongiform encephalopathy ( BSE ) has not been reported in Austria , the data do not support a link between a rise in incidence of sporadic CJD and BSE .
	manualset3
241563	3	423706	15	NULL	NULL	0	NULL	data 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	As bovine spongiform encephalopathy ( BSE ) has not been reported in Austria , the data do not support a link between a rise in incidence of sporadic CJD and BSE .
	manualset3
241564	4	423706	15	NULL	NULL	0	NULL	support 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As bovine spongiform encephalopathy ( BSE ) has not been reported in Austria , the data do not support a link between a rise in incidence of sporadic CJD and BSE .
	manualset3
241565	5	423706	15	NULL	NULL	0	NULL	link 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	As bovine spongiform encephalopathy ( BSE ) has not been reported in Austria , the data do not support a link between a rise in incidence of sporadic CJD and BSE .
	manualset3
241566	6	423706	15	NULL	NULL	0	NULL	rise in incidence of sporadic CJD 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As bovine spongiform encephalopathy ( BSE ) has not been reported in Austria , the data do not support a link between a rise in incidence of sporadic CJD and BSE .
	manualset3
241567	7	423706	15	NULL	NULL	0	NULL	rise in incidence of sporadic BSE 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As bovine spongiform encephalopathy ( BSE ) has not been reported in Austria , the data do not support a link between a rise in incidence of sporadic CJD and BSE .
	manualset3
241568	1	423707	15	NULL	NULL	NULL	NULL	 unanesthetized state	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As compared to the unanesthetized state , each of these agents has some influence on CBF and metabolism , and many have significant effects on vascular responses to dilator stimuli .
	manualset3
241569	2	423707	15	NULL	NULL	0	NULL	agents	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As compared to the unanesthetized state , each of these agents has some influence on CBF and metabolism , and many have significant effects on vascular responses to dilator stimuli .
	manualset3
241570	3	423707	15	NULL	NULL	0	NULL	influence on CBF	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As compared to the unanesthetized state , each of these agents has some influence on CBF and metabolism , and many have significant effects on vascular responses to dilator stimuli .
	manualset3
241572	4	423707	15	NULL	NULL	NULL	NULL	influence on metabolism	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As compared to the unanesthetized state , each of these agents has some influence on CBF and metabolism , and many have significant effects on vascular responses to dilator stimuli .
	manualset3
241575	5	423707	15	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As compared to the unanesthetized state , each of these agents has some influence on CBF and metabolism , and many have significant effects on vascular responses to dilator stimuli .
	manualset3
241576	6	423707	15	NULL	NULL	0	NULL	vascular responses to dilator stimuli 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As compared to the unanesthetized state , each of these agents has some influence on CBF and metabolism , and many have significant effects on vascular responses to dilator stimuli .
	manualset3
241589	1	423708	15	NULL	NULL	NULL	NULL	control ( without coculture with osteoclasts )	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As compared with control ( without coculture with osteoclasts ) , the viability of MM cells cocultured with osteoclasts obviously increased , the expression levels of c-jun , junD , fos and fosB decreased to 25.7 % - 1.66 % , 68.49 % - 8.54 % , 10.35 % - 0.19 % and 36.63 % - 3.44 % of the control respectively .
	manualset3
241594	2	423708	15	NULL	NULL	0	NULL	viability of MM cells	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As compared with control ( without coculture with osteoclasts ) , the viability of MM cells cocultured with osteoclasts obviously increased , the expression levels of c-jun , junD , fos and fosB decreased to 25.7 % - 1.66 % , 68.49 % - 8.54 % , 10.35 % - 0.19 % and 36.63 % - 3.44 % of the control respectively .
	manualset3
241596	3	423708	15	NULL	NULL	0	NULL	osteoclasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	As compared with control ( without coculture with osteoclasts ) , the viability of MM cells cocultured with osteoclasts obviously increased , the expression levels of c-jun , junD , fos and fosB decreased to 25.7 % - 1.66 % , 68.49 % - 8.54 % , 10.35 % - 0.19 % and 36.63 % - 3.44 % of the control respectively .
	manualset3
241597	4	423708	15	NULL	NULL	NULL	NULL	expression levels of c-jun	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As compared with control ( without coculture with osteoclasts ) , the viability of MM cells cocultured with osteoclasts obviously increased , the expression levels of c-jun , junD , fos and fosB decreased to 25.7 % - 1.66 % , 68.49 % - 8.54 % , 10.35 % - 0.19 % and 36.63 % - 3.44 % of the control respectively .
	manualset3
241598	5	423708	15	NULL	NULL	NULL	NULL	expression levels of junD	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As compared with control ( without coculture with osteoclasts ) , the viability of MM cells cocultured with osteoclasts obviously increased , the expression levels of c-jun , junD , fos and fosB decreased to 25.7 % - 1.66 % , 68.49 % - 8.54 % , 10.35 % - 0.19 % and 36.63 % - 3.44 % of the control respectively .
	manualset3
241599	6	423708	15	NULL	NULL	NULL	NULL	expression levels of fos	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As compared with control ( without coculture with osteoclasts ) , the viability of MM cells cocultured with osteoclasts obviously increased , the expression levels of c-jun , junD , fos and fosB decreased to 25.7 % - 1.66 % , 68.49 % - 8.54 % , 10.35 % - 0.19 % and 36.63 % - 3.44 % of the control respectively .
	manualset3
241601	7	423708	15	NULL	NULL	NULL	NULL	expression levels of fosB 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As compared with control ( without coculture with osteoclasts ) , the viability of MM cells cocultured with osteoclasts obviously increased , the expression levels of c-jun , junD , fos and fosB decreased to 25.7 % - 1.66 % , 68.49 % - 8.54 % , 10.35 % - 0.19 % and 36.63 % - 3.44 % of the control respectively .
	manualset3
241611	8	423708	15	NULL	NULL	0	NULL	25.7 % - 1.66 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As compared with control ( without coculture with osteoclasts ) , the viability of MM cells cocultured with osteoclasts obviously increased , the expression levels of c-jun , junD , fos and fosB decreased to 25.7 % - 1.66 % , 68.49 % - 8.54 % , 10.35 % - 0.19 % and 36.63 % - 3.44 % of the control respectively .
	manualset3
241613	9	423708	15	NULL	NULL	0	NULL	68.49 % - 8.54 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As compared with control ( without coculture with osteoclasts ) , the viability of MM cells cocultured with osteoclasts obviously increased , the expression levels of c-jun , junD , fos and fosB decreased to 25.7 % - 1.66 % , 68.49 % - 8.54 % , 10.35 % - 0.19 % and 36.63 % - 3.44 % of the control respectively .
	manualset3
241614	10	423708	15	NULL	NULL	0	NULL	10.35 % - 0.19 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As compared with control ( without coculture with osteoclasts ) , the viability of MM cells cocultured with osteoclasts obviously increased , the expression levels of c-jun , junD , fos and fosB decreased to 25.7 % - 1.66 % , 68.49 % - 8.54 % , 10.35 % - 0.19 % and 36.63 % - 3.44 % of the control respectively .
	manualset3
241616	11	423708	15	NULL	NULL	0	NULL	36.63 % - 3.44 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As compared with control ( without coculture with osteoclasts ) , the viability of MM cells cocultured with osteoclasts obviously increased , the expression levels of c-jun , junD , fos and fosB decreased to 25.7 % - 1.66 % , 68.49 % - 8.54 % , 10.35 % - 0.19 % and 36.63 % - 3.44 % of the control respectively .
	manualset3
241617	12	423708	15	NULL	NULL	0	NULL	control	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	As compared with control ( without coculture with osteoclasts ) , the viability of MM cells cocultured with osteoclasts obviously increased , the expression levels of c-jun , junD , fos and fosB decreased to 25.7 % - 1.66 % , 68.49 % - 8.54 % , 10.35 % - 0.19 % and 36.63 % - 3.44 % of the control respectively .
	manualset3
241625	1	423709	15	NULL	NULL	NULL	NULL	tertile	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As compared with the first tertile , the age - and sex-adjusted hazard ratios ( 95 % confidence intervals ) for all-cause mortality , CVD events and CHD events were 1.30 ( 0.92-1 .83 ) , 1.40 ( 1.09-1 .81 ) and 2.04 ( 1.35-3 .10 ) , respectively , for subjects in the upper tertile of ALT .
	manualset3
241627	2	423709	15	NULL	NULL	0	NULL	age adjusted hazard ratios 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As compared with the first tertile , the age - and sex-adjusted hazard ratios ( 95 % confidence intervals ) for all-cause mortality , CVD events and CHD events were 1.30 ( 0.92-1 .83 ) , 1.40 ( 1.09-1 .81 ) and 2.04 ( 1.35-3 .10 ) , respectively , for subjects in the upper tertile of ALT .
	manualset3
241629	3	423709	15	NULL	NULL	0	NULL	sex-adjusted hazard ratios	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As compared with the first tertile , the age - and sex-adjusted hazard ratios ( 95 % confidence intervals ) for all-cause mortality , CVD events and CHD events were 1.30 ( 0.92-1 .83 ) , 1.40 ( 1.09-1 .81 ) and 2.04 ( 1.35-3 .10 ) , respectively , for subjects in the upper tertile of ALT .
	manualset3
241630	4	423709	15	NULL	NULL	0	NULL	95 % confidence intervals	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As compared with the first tertile , the age - and sex-adjusted hazard ratios ( 95 % confidence intervals ) for all-cause mortality , CVD events and CHD events were 1.30 ( 0.92-1 .83 ) , 1.40 ( 1.09-1 .81 ) and 2.04 ( 1.35-3 .10 ) , respectively , for subjects in the upper tertile of ALT .
	manualset3
241634	5	423709	15	NULL	NULL	0	NULL	all-cause mortality 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As compared with the first tertile , the age - and sex-adjusted hazard ratios ( 95 % confidence intervals ) for all-cause mortality , CVD events and CHD events were 1.30 ( 0.92-1 .83 ) , 1.40 ( 1.09-1 .81 ) and 2.04 ( 1.35-3 .10 ) , respectively , for subjects in the upper tertile of ALT .
	manualset3
241635	6	423709	15	NULL	NULL	0	NULL	CVD events	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As compared with the first tertile , the age - and sex-adjusted hazard ratios ( 95 % confidence intervals ) for all-cause mortality , CVD events and CHD events were 1.30 ( 0.92-1 .83 ) , 1.40 ( 1.09-1 .81 ) and 2.04 ( 1.35-3 .10 ) , respectively , for subjects in the upper tertile of ALT .
	manualset3
241637	7	423709	15	NULL	NULL	0	NULL	CHD events 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As compared with the first tertile , the age - and sex-adjusted hazard ratios ( 95 % confidence intervals ) for all-cause mortality , CVD events and CHD events were 1.30 ( 0.92-1 .83 ) , 1.40 ( 1.09-1 .81 ) and 2.04 ( 1.35-3 .10 ) , respectively , for subjects in the upper tertile of ALT .
	manualset3
241641	8	423709	15	NULL	NULL	NULL	NULL	1.30 ( 0.92-1 .83 )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As compared with the first tertile , the age - and sex-adjusted hazard ratios ( 95 % confidence intervals ) for all-cause mortality , CVD events and CHD events were 1.30 ( 0.92-1 .83 ) , 1.40 ( 1.09-1 .81 ) and 2.04 ( 1.35-3 .10 ) , respectively , for subjects in the upper tertile of ALT .
	manualset3
241642	9	423709	15	NULL	NULL	NULL	NULL	1.40 ( 1.09-1 .81 )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As compared with the first tertile , the age - and sex-adjusted hazard ratios ( 95 % confidence intervals ) for all-cause mortality , CVD events and CHD events were 1.30 ( 0.92-1 .83 ) , 1.40 ( 1.09-1 .81 ) and 2.04 ( 1.35-3 .10 ) , respectively , for subjects in the upper tertile of ALT .
	manualset3
241643	10	423709	15	NULL	NULL	NULL	NULL	2.04 ( 1.35-3 .10 )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As compared with the first tertile , the age - and sex-adjusted hazard ratios ( 95 % confidence intervals ) for all-cause mortality , CVD events and CHD events were 1.30 ( 0.92-1 .83 ) , 1.40 ( 1.09-1 .81 ) and 2.04 ( 1.35-3 .10 ) , respectively , for subjects in the upper tertile of ALT .
	manualset3
241644	11	423709	15	NULL	NULL	0	NULL	subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As compared with the first tertile , the age - and sex-adjusted hazard ratios ( 95 % confidence intervals ) for all-cause mortality , CVD events and CHD events were 1.30 ( 0.92-1 .83 ) , 1.40 ( 1.09-1 .81 ) and 2.04 ( 1.35-3 .10 ) , respectively , for subjects in the upper tertile of ALT .
	manualset3
241645	12	423709	15	NULL	NULL	NULL	NULL	tertile of ALT	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As compared with the first tertile , the age - and sex-adjusted hazard ratios ( 95 % confidence intervals ) for all-cause mortality , CVD events and CHD events were 1.30 ( 0.92-1 .83 ) , 1.40 ( 1.09-1 .81 ) and 2.04 ( 1.35-3 .10 ) , respectively , for subjects in the upper tertile of ALT .
	manualset3
241651	1	423710	15	NULL	NULL	0	NULL	congeners 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	As coplanar congeners show a higher affinity for Florisil , 20 ml of hexane-dichloromethane ( 90 : 10 ) were necessary for the quantitative recovery of coplanar and non-coplanar CBs .
	manualset3
241653	3	423710	15	NULL	NULL	NULL	NULL	Florisil	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As coplanar congeners show a higher affinity for Florisil , 20 ml of hexane-dichloromethane ( 90 : 10 ) were necessary for the quantitative recovery of coplanar and non-coplanar CBs .
	manualset3
241654	4	423710	15	NULL	NULL	NULL	NULL	20 ml of hexane-dichloromethane ( 90 : 10 ) 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As coplanar congeners show a higher affinity for Florisil , 20 ml of hexane-dichloromethane ( 90 : 10 ) were necessary for the quantitative recovery of coplanar and non-coplanar CBs .
	manualset3
241655	5	423710	15	NULL	NULL	NULL	NULL	quantitative recovery of coplanar CBs  	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As coplanar congeners show a higher affinity for Florisil , 20 ml of hexane-dichloromethane ( 90 : 10 ) were necessary for the quantitative recovery of coplanar and non-coplanar CBs .
	manualset3
241656	6	423710	15	NULL	NULL	NULL	NULL	quantitative recovery of non-coplanar CBs	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As coplanar congeners show a higher affinity for Florisil , 20 ml of hexane-dichloromethane ( 90 : 10 ) were necessary for the quantitative recovery of coplanar and non-coplanar CBs .
	manualset3
241657	2	423710	15	NULL	NULL	NULL	NULL	 affinity 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As coplanar congeners show a higher affinity for Florisil , 20 ml of hexane-dichloromethane ( 90 : 10 ) were necessary for the quantitative recovery of coplanar and non-coplanar CBs .
	manualset3
241658	1	423711	15	NULL	NULL	0	NULL	duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	As duration of inflammatory bowel disease ( IBD ) , in particular ulcerative colitis ( UC ) , is a major risk factor for the development of colorectal cancer ( CRC ) , it is rational to propose a screening colonoscopy when the risk starts to increase , i.e. , after 8-10 years from the onset of disease .
	manualset3
241659	2	423711	15	NULL	NULL	0	NULL	inflammatory bowel disease ( IBD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	As duration of inflammatory bowel disease ( IBD ) , in particular ulcerative colitis ( UC ) , is a major risk factor for the development of colorectal cancer ( CRC ) , it is rational to propose a screening colonoscopy when the risk starts to increase , i.e. , after 8-10 years from the onset of disease .
	manualset3
241660	3	423711	15	NULL	NULL	0	NULL	ulcerative colitis ( UC ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	As duration of inflammatory bowel disease ( IBD ) , in particular ulcerative colitis ( UC ) , is a major risk factor for the development of colorectal cancer ( CRC ) , it is rational to propose a screening colonoscopy when the risk starts to increase , i.e. , after 8-10 years from the onset of disease .
	manualset3
241661	4	423711	15	NULL	NULL	0	NULL	risk factor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As duration of inflammatory bowel disease ( IBD ) , in particular ulcerative colitis ( UC ) , is a major risk factor for the development of colorectal cancer ( CRC ) , it is rational to propose a screening colonoscopy when the risk starts to increase , i.e. , after 8-10 years from the onset of disease .
	manualset3
241662	5	423711	15	NULL	NULL	0	NULL	development of colorectal cancer ( CRC )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As duration of inflammatory bowel disease ( IBD ) , in particular ulcerative colitis ( UC ) , is a major risk factor for the development of colorectal cancer ( CRC ) , it is rational to propose a screening colonoscopy when the risk starts to increase , i.e. , after 8-10 years from the onset of disease .
	manualset3
241663	6	423711	15	NULL	NULL	0	NULL	screening colonoscopy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As duration of inflammatory bowel disease ( IBD ) , in particular ulcerative colitis ( UC ) , is a major risk factor for the development of colorectal cancer ( CRC ) , it is rational to propose a screening colonoscopy when the risk starts to increase , i.e. , after 8-10 years from the onset of disease .
	manualset3
241664	7	423711	15	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As duration of inflammatory bowel disease ( IBD ) , in particular ulcerative colitis ( UC ) , is a major risk factor for the development of colorectal cancer ( CRC ) , it is rational to propose a screening colonoscopy when the risk starts to increase , i.e. , after 8-10 years from the onset of disease .
	manualset3
241665	8	423711	15	NULL	NULL	0	NULL	increase 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As duration of inflammatory bowel disease ( IBD ) , in particular ulcerative colitis ( UC ) , is a major risk factor for the development of colorectal cancer ( CRC ) , it is rational to propose a screening colonoscopy when the risk starts to increase , i.e. , after 8-10 years from the onset of disease .
	manualset3
241666	9	423711	15	NULL	NULL	0	NULL	 8-10 years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	As duration of inflammatory bowel disease ( IBD ) , in particular ulcerative colitis ( UC ) , is a major risk factor for the development of colorectal cancer ( CRC ) , it is rational to propose a screening colonoscopy when the risk starts to increase , i.e. , after 8-10 years from the onset of disease .
	manualset3
241667	10	423711	15	NULL	NULL	0	NULL	onset of disease	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As duration of inflammatory bowel disease ( IBD ) , in particular ulcerative colitis ( UC ) , is a major risk factor for the development of colorectal cancer ( CRC ) , it is rational to propose a screening colonoscopy when the risk starts to increase , i.e. , after 8-10 years from the onset of disease .
	manualset3
241668	1	423712	15	NULL	NULL	NULL	NULL	tropomyosin subunit	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As each tropomyosin subunit formed two precipitin lines with the homologous antiserum , as many as ten kinds of subunits may exist in chicken muscles .
	manualset3
241669	2	423712	15	NULL	NULL	0	NULL	two precipitin lines	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	As each tropomyosin subunit formed two precipitin lines with the homologous antiserum , as many as ten kinds of subunits may exist in chicken muscles .
	manualset3
241670	3	423712	15	NULL	NULL	NULL	NULL	homologous antiserum	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As each tropomyosin subunit formed two precipitin lines with the homologous antiserum , as many as ten kinds of subunits may exist in chicken muscles .
	manualset3
241671	4	423712	15	NULL	NULL	0	NULL	ten kinds of subunits	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	As each tropomyosin subunit formed two precipitin lines with the homologous antiserum , as many as ten kinds of subunits may exist in chicken muscles .
	manualset3
241672	5	423712	15	NULL	NULL	0	NULL	chicken muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	As each tropomyosin subunit formed two precipitin lines with the homologous antiserum , as many as ten kinds of subunits may exist in chicken muscles .
	manualset3
241673	1	423713	15	NULL	NULL	0	NULL	attempts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As few attempts have been made to distinguish free 5 ' ends of true replicate from those of abortive ones , we examined the 5 ' ends of true replicate of human mitochondrial DNA at one nucleotide resolution in vivo by making use of ligation-mediated polymerase chain reaction .
	manualset3
241674	2	423713	15	NULL	NULL	0	NULL	free 5 ' ends of true replicate	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	As few attempts have been made to distinguish free 5 ' ends of true replicate from those of abortive ones , we examined the 5 ' ends of true replicate of human mitochondrial DNA at one nucleotide resolution in vivo by making use of ligation-mediated polymerase chain reaction .
	manualset3
241675	3	423713	15	NULL	NULL	0	NULL	abortive ones	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	As few attempts have been made to distinguish free 5 ' ends of true replicate from those of abortive ones , we examined the 5 ' ends of true replicate of human mitochondrial DNA at one nucleotide resolution in vivo by making use of ligation-mediated polymerase chain reaction .
	manualset3
241676	4	423713	15	NULL	NULL	0	NULL	5 ' ends of true replicate of human mitochondrial DNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	As few attempts have been made to distinguish free 5 ' ends of true replicate from those of abortive ones , we examined the 5 ' ends of true replicate of human mitochondrial DNA at one nucleotide resolution in vivo by making use of ligation-mediated polymerase chain reaction .
	manualset3
241677	5	423713	15	NULL	NULL	NULL	NULL	one nucleotide resolution	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As few attempts have been made to distinguish free 5 ' ends of true replicate from those of abortive ones , we examined the 5 ' ends of true replicate of human mitochondrial DNA at one nucleotide resolution in vivo by making use of ligation-mediated polymerase chain reaction .
	manualset3
241679	6	423713	15	NULL	NULL	NULL	NULL	ligation-mediated polymerase chain reaction	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As few attempts have been made to distinguish free 5 ' ends of true replicate from those of abortive ones , we examined the 5 ' ends of true replicate of human mitochondrial DNA at one nucleotide resolution in vivo by making use of ligation-mediated polymerase chain reaction .
	manualset3
241921	1	423714	15	NULL	NULL	NULL	NULL	glucagon release	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As for glucagon release , the response to arginine was not inhibited normally by glucose , resulting in threefold higher levels at 11 mmol/l glucose versus control subjects .
	manualset3
241922	2	423714	15	NULL	NULL	0	NULL	response to arginine 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As for glucagon release , the response to arginine was not inhibited normally by glucose , resulting in threefold higher levels at 11 mmol/l glucose versus control subjects .
	manualset3
241923	3	423714	15	NULL	NULL	0	NULL	glucose 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	As for glucagon release , the response to arginine was not inhibited normally by glucose , resulting in threefold higher levels at 11 mmol/l glucose versus control subjects .
	manualset3
241924	4	423714	15	NULL	NULL	0	NULL	threefold	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	As for glucagon release , the response to arginine was not inhibited normally by glucose , resulting in threefold higher levels at 11 mmol/l glucose versus control subjects .
	manualset3
241925	5	423714	15	NULL	NULL	0	NULL	levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As for glucagon release , the response to arginine was not inhibited normally by glucose , resulting in threefold higher levels at 11 mmol/l glucose versus control subjects .
	manualset3
241926	6	423714	15	NULL	NULL	0	NULL	11 mmol/l glucose 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As for glucagon release , the response to arginine was not inhibited normally by glucose , resulting in threefold higher levels at 11 mmol/l glucose versus control subjects .
	manualset3
241927	7	423714	15	NULL	NULL	0	NULL	control subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As for glucagon release , the response to arginine was not inhibited normally by glucose , resulting in threefold higher levels at 11 mmol/l glucose versus control subjects .
	manualset3
242060	1	423715	15	NULL	NULL	0	NULL	mALP 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	As for mALP , the result suggested that post-translational modification was important for the proteins to express activity and to represent their extensive polymorphic nature , whereas the magnitude of activities was mainly regulated by transcription .
	manualset3
242061	2	423715	15	NULL	NULL	0	NULL	result 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	As for mALP , the result suggested that post-translational modification was important for the proteins to express activity and to represent their extensive polymorphic nature , whereas the magnitude of activities was mainly regulated by transcription .
	manualset3
242062	3	423715	15	NULL	NULL	0	NULL	post-translational modification	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As for mALP , the result suggested that post-translational modification was important for the proteins to express activity and to represent their extensive polymorphic nature , whereas the magnitude of activities was mainly regulated by transcription .
	manualset3
242063	4	423715	15	NULL	NULL	0	NULL	proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	As for mALP , the result suggested that post-translational modification was important for the proteins to express activity and to represent their extensive polymorphic nature , whereas the magnitude of activities was mainly regulated by transcription .
	manualset3
242064	5	423715	15	NULL	NULL	0	NULL	activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As for mALP , the result suggested that post-translational modification was important for the proteins to express activity and to represent their extensive polymorphic nature , whereas the magnitude of activities was mainly regulated by transcription .
	manualset3
242066	6	423715	15	NULL	NULL	0	NULL	extensive polymorphic nature	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As for mALP , the result suggested that post-translational modification was important for the proteins to express activity and to represent their extensive polymorphic nature , whereas the magnitude of activities was mainly regulated by transcription .
	manualset3
242067	7	423715	15	NULL	NULL	0	NULL	magnitude of activities	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As for mALP , the result suggested that post-translational modification was important for the proteins to express activity and to represent their extensive polymorphic nature , whereas the magnitude of activities was mainly regulated by transcription .
	manualset3
242068	8	423715	15	NULL	NULL	0	NULL	transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As for mALP , the result suggested that post-translational modification was important for the proteins to express activity and to represent their extensive polymorphic nature , whereas the magnitude of activities was mainly regulated by transcription .
	manualset3
241928	1	423716	15	NULL	NULL	0	NULL	motion estimation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As for motion estimation , we minimize an objective function involving two robust terms .
	manualset3
241929	2	423716	15	NULL	NULL	0	NULL	objective function 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As for motion estimation , we minimize an objective function involving two robust terms .
	manualset3
241930	3	423716	15	NULL	NULL	0	NULL	two 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	As for motion estimation , we minimize an objective function involving two robust terms .
	manualset3
241931	4	423716	15	NULL	NULL	0	NULL	robust terms 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As for motion estimation , we minimize an objective function involving two robust terms .
	manualset3
241932	1	423717	15	NULL	NULL	0	NULL	health policies	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	As future health policies develop , the appropriate types and levels of nutrition services are important to consider .
	manualset3
241933	2	423717	15	NULL	NULL	0	NULL	types	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As future health policies develop , the appropriate types and levels of nutrition services are important to consider .
	manualset3
241934	3	423717	15	NULL	NULL	0	NULL	levels of nutrition services 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As future health policies develop , the appropriate types and levels of nutrition services are important to consider .
	manualset3
241937	1	423718	15	NULL	NULL	0	NULL	metastases	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As her metastases were controlled for about 7 months , hepatic arterial infusion of mitomycin C and degradable starch microspheres appears to be useful for treating liver metastasis of pancreatic cancer , but careful attention should be paid to the risk of severe complications such as bile duct necrosis .
	manualset3
241938	2	423718	15	NULL	NULL	0	NULL	7 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	As her metastases were controlled for about 7 months , hepatic arterial infusion of mitomycin C and degradable starch microspheres appears to be useful for treating liver metastasis of pancreatic cancer , but careful attention should be paid to the risk of severe complications such as bile duct necrosis .
	manualset3
241939	3	423718	15	NULL	NULL	0	NULL	hepatic arterial infusion 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As her metastases were controlled for about 7 months , hepatic arterial infusion of mitomycin C and degradable starch microspheres appears to be useful for treating liver metastasis of pancreatic cancer , but careful attention should be paid to the risk of severe complications such as bile duct necrosis .
	manualset3
241940	4	423718	15	NULL	NULL	0	NULL	mitomycin C 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	As her metastases were controlled for about 7 months , hepatic arterial infusion of mitomycin C and degradable starch microspheres appears to be useful for treating liver metastasis of pancreatic cancer , but careful attention should be paid to the risk of severe complications such as bile duct necrosis .
	manualset3
241941	5	423718	15	NULL	NULL	0	NULL	degradable starch microspheres 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	As her metastases were controlled for about 7 months , hepatic arterial infusion of mitomycin C and degradable starch microspheres appears to be useful for treating liver metastasis of pancreatic cancer , but careful attention should be paid to the risk of severe complications such as bile duct necrosis .
	manualset3
241942	6	423718	15	NULL	NULL	0	NULL	treating liver metastasis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As her metastases were controlled for about 7 months , hepatic arterial infusion of mitomycin C and degradable starch microspheres appears to be useful for treating liver metastasis of pancreatic cancer , but careful attention should be paid to the risk of severe complications such as bile duct necrosis .
	manualset3
241943	7	423718	15	NULL	NULL	0	NULL	pancreatic cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	As her metastases were controlled for about 7 months , hepatic arterial infusion of mitomycin C and degradable starch microspheres appears to be useful for treating liver metastasis of pancreatic cancer , but careful attention should be paid to the risk of severe complications such as bile duct necrosis .
	manualset3
241945	8	423718	15	NULL	NULL	0	NULL	attention	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As her metastases were controlled for about 7 months , hepatic arterial infusion of mitomycin C and degradable starch microspheres appears to be useful for treating liver metastasis of pancreatic cancer , but careful attention should be paid to the risk of severe complications such as bile duct necrosis .
	manualset3
241947	9	423718	15	NULL	NULL	0	NULL	risk of severe complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As her metastases were controlled for about 7 months , hepatic arterial infusion of mitomycin C and degradable starch microspheres appears to be useful for treating liver metastasis of pancreatic cancer , but careful attention should be paid to the risk of severe complications such as bile duct necrosis .
	manualset3
241949	10	423718	15	NULL	NULL	0	NULL	bile duct necrosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As her metastases were controlled for about 7 months , hepatic arterial infusion of mitomycin C and degradable starch microspheres appears to be useful for treating liver metastasis of pancreatic cancer , but careful attention should be paid to the risk of severe complications such as bile duct necrosis .
	manualset3
241970	1	423719	15	NULL	NULL	0	NULL	eutherian mammals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	As in eutherian mammals , OT-like peptides are distributed throughout the brain and are present in the testis , corpus luteum , prostate and adrenal glands .
	manualset3
241971	2	423719	15	NULL	NULL	0	NULL	OT-like peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	As in eutherian mammals , OT-like peptides are distributed throughout the brain and are present in the testis , corpus luteum , prostate and adrenal glands .
	manualset3
241972	3	423719	15	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	As in eutherian mammals , OT-like peptides are distributed throughout the brain and are present in the testis , corpus luteum , prostate and adrenal glands .
	manualset3
241973	4	423719	15	NULL	NULL	0	NULL	testis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	As in eutherian mammals , OT-like peptides are distributed throughout the brain and are present in the testis , corpus luteum , prostate and adrenal glands .
	manualset3
241974	5	423719	15	NULL	NULL	0	NULL	corpus luteum 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	As in eutherian mammals , OT-like peptides are distributed throughout the brain and are present in the testis , corpus luteum , prostate and adrenal glands .
	manualset3
241975	6	423719	15	NULL	NULL	0	NULL	prostate	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	As in eutherian mammals , OT-like peptides are distributed throughout the brain and are present in the testis , corpus luteum , prostate and adrenal glands .
	manualset3
241976	7	423719	15	NULL	NULL	0	NULL	adrenal glands	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	As in eutherian mammals , OT-like peptides are distributed throughout the brain and are present in the testis , corpus luteum , prostate and adrenal glands .
	manualset3
241979	1	423720	15	NULL	NULL	0	NULL	bacterial ribosome	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	As in the bacterial ribosome , bridges between the subunits are mainly formed by RNA contacts .
	manualset3
241981	2	423720	15	NULL	NULL	0	NULL	bridges 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	As in the bacterial ribosome , bridges between the subunits are mainly formed by RNA contacts .
	manualset3
241983	3	423720	15	NULL	NULL	0	NULL	subunits	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	As in the bacterial ribosome , bridges between the subunits are mainly formed by RNA contacts .
	manualset3
241986	4	423720	15	NULL	NULL	0	NULL	RNA contacts	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	As in the bacterial ribosome , bridges between the subunits are mainly formed by RNA contacts .
	manualset3
241990	1	423721	15	NULL	NULL	0	NULL	case of epilepsy	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	As in the case of epilepsy , depression and pain syndromes have a relatively high comorbidity .
	manualset3
241992	2	423721	15	NULL	NULL	0	NULL	depression	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As in the case of epilepsy , depression and pain syndromes have a relatively high comorbidity .
	manualset3
241993	3	423721	15	NULL	NULL	0	NULL	pain syndromes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As in the case of epilepsy , depression and pain syndromes have a relatively high comorbidity .
	manualset3
241996	4	423721	15	NULL	NULL	0	NULL	comorbidity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As in the case of epilepsy , depression and pain syndromes have a relatively high comorbidity .
	manualset3
241998	1	423722	15	NULL	NULL	0	NULL	managers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As managers of the pediatric medical home and advocates for children and optimal pediatric health care , there is a very important role for pediatricians and the American Academy of Pediatrics in guiding health policy decision-makers toward effective solutions that promote the medical home and timely access to emergency care .
	manualset3
241999	2	423722	15	NULL	NULL	0	NULL	pediatric medical home	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	As managers of the pediatric medical home and advocates for children and optimal pediatric health care , there is a very important role for pediatricians and the American Academy of Pediatrics in guiding health policy decision-makers toward effective solutions that promote the medical home and timely access to emergency care .
	manualset3
242000	3	423722	15	NULL	NULL	0	NULL	advocates 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As managers of the pediatric medical home and advocates for children and optimal pediatric health care , there is a very important role for pediatricians and the American Academy of Pediatrics in guiding health policy decision-makers toward effective solutions that promote the medical home and timely access to emergency care .
	manualset3
242001	4	423722	15	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As managers of the pediatric medical home and advocates for children and optimal pediatric health care , there is a very important role for pediatricians and the American Academy of Pediatrics in guiding health policy decision-makers toward effective solutions that promote the medical home and timely access to emergency care .
	manualset3
242002	5	423722	15	NULL	NULL	0	NULL	optimal pediatric health care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As managers of the pediatric medical home and advocates for children and optimal pediatric health care , there is a very important role for pediatricians and the American Academy of Pediatrics in guiding health policy decision-makers toward effective solutions that promote the medical home and timely access to emergency care .
	manualset3
242003	6	423722	15	NULL	NULL	0	NULL	role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As managers of the pediatric medical home and advocates for children and optimal pediatric health care , there is a very important role for pediatricians and the American Academy of Pediatrics in guiding health policy decision-makers toward effective solutions that promote the medical home and timely access to emergency care .
	manualset3
242004	7	423722	15	NULL	NULL	0	NULL	pediatricians 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As managers of the pediatric medical home and advocates for children and optimal pediatric health care , there is a very important role for pediatricians and the American Academy of Pediatrics in guiding health policy decision-makers toward effective solutions that promote the medical home and timely access to emergency care .
	manualset3
242007	8	423722	15	NULL	NULL	0	NULL	American Academy of Pediatrics	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	As managers of the pediatric medical home and advocates for children and optimal pediatric health care , there is a very important role for pediatricians and the American Academy of Pediatrics in guiding health policy decision-makers toward effective solutions that promote the medical home and timely access to emergency care .
	manualset3
242008	9	423722	15	NULL	NULL	0	NULL	health policy decision-makers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As managers of the pediatric medical home and advocates for children and optimal pediatric health care , there is a very important role for pediatricians and the American Academy of Pediatrics in guiding health policy decision-makers toward effective solutions that promote the medical home and timely access to emergency care .
	manualset3
242009	10	423722	15	NULL	NULL	0	NULL	solutions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As managers of the pediatric medical home and advocates for children and optimal pediatric health care , there is a very important role for pediatricians and the American Academy of Pediatrics in guiding health policy decision-makers toward effective solutions that promote the medical home and timely access to emergency care .
	manualset3
242010	11	423722	15	NULL	NULL	0	NULL	medical home	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	As managers of the pediatric medical home and advocates for children and optimal pediatric health care , there is a very important role for pediatricians and the American Academy of Pediatrics in guiding health policy decision-makers toward effective solutions that promote the medical home and timely access to emergency care .
	manualset3
242012	12	423722	15	NULL	NULL	0	NULL	access	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As managers of the pediatric medical home and advocates for children and optimal pediatric health care , there is a very important role for pediatricians and the American Academy of Pediatrics in guiding health policy decision-makers toward effective solutions that promote the medical home and timely access to emergency care .
	manualset3
242014	13	423722	15	NULL	NULL	0	NULL	emergency care	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	As managers of the pediatric medical home and advocates for children and optimal pediatric health care , there is a very important role for pediatricians and the American Academy of Pediatrics in guiding health policy decision-makers toward effective solutions that promote the medical home and timely access to emergency care .
	manualset3
242050	1	423723	15	NULL	NULL	0	NULL	measures for p ( EXL ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As measures for p ( EXL ) the mean lifetime concentration of SO in the transitional zone of the lung and for p ( HPS ) the mean lifetime concentration of SO in blood were calculated using a physiological toxicokinetic model .
	manualset3
242052	2	423723	15	NULL	NULL	0	NULL	mean lifetime concentration 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As measures for p ( EXL ) the mean lifetime concentration of SO in the transitional zone of the lung and for p ( HPS ) the mean lifetime concentration of SO in blood were calculated using a physiological toxicokinetic model .
	manualset3
242053	3	423723	15	NULL	NULL	0	NULL	SO 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	As measures for p ( EXL ) the mean lifetime concentration of SO in the transitional zone of the lung and for p ( HPS ) the mean lifetime concentration of SO in blood were calculated using a physiological toxicokinetic model .
	manualset3
242054	4	423723	15	NULL	NULL	0	NULL	transitional zone of the lung	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	As measures for p ( EXL ) the mean lifetime concentration of SO in the transitional zone of the lung and for p ( HPS ) the mean lifetime concentration of SO in blood were calculated using a physiological toxicokinetic model .
	manualset3
242055	5	423723	15	NULL	NULL	0	NULL	p ( HPS )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As measures for p ( EXL ) the mean lifetime concentration of SO in the transitional zone of the lung and for p ( HPS ) the mean lifetime concentration of SO in blood were calculated using a physiological toxicokinetic model .
	manualset3
242056	6	423723	15	NULL	NULL	0	NULL	mean lifetime concentration 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As measures for p ( EXL ) the mean lifetime concentration of SO in the transitional zone of the lung and for p ( HPS ) the mean lifetime concentration of SO in blood were calculated using a physiological toxicokinetic model .
	manualset3
242057	7	423723	15	NULL	NULL	0	NULL	SO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	As measures for p ( EXL ) the mean lifetime concentration of SO in the transitional zone of the lung and for p ( HPS ) the mean lifetime concentration of SO in blood were calculated using a physiological toxicokinetic model .
	manualset3
242058	8	423723	15	NULL	NULL	0	NULL	blood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	As measures for p ( EXL ) the mean lifetime concentration of SO in the transitional zone of the lung and for p ( HPS ) the mean lifetime concentration of SO in blood were calculated using a physiological toxicokinetic model .
	manualset3
242059	9	423723	15	NULL	NULL	0	NULL	physiological toxicokinetic model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	As measures for p ( EXL ) the mean lifetime concentration of SO in the transitional zone of the lung and for p ( HPS ) the mean lifetime concentration of SO in blood were calculated using a physiological toxicokinetic model .
	manualset3
242070	1	423724	15	NULL	NULL	0	NULL	studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	As not many studies with phytase have been performed during gestation and lactation in sows yet , we can recommend , that phytase as supplement can be used to keep P in the diet at a lower level without negative consequences for bone health .
	manualset3
242071	2	423724	15	NULL	NULL	0	NULL	phytase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	As not many studies with phytase have been performed during gestation and lactation in sows yet , we can recommend , that phytase as supplement can be used to keep P in the diet at a lower level without negative consequences for bone health .
	manualset3
242072	3	423724	15	NULL	NULL	0	NULL	gestation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As not many studies with phytase have been performed during gestation and lactation in sows yet , we can recommend , that phytase as supplement can be used to keep P in the diet at a lower level without negative consequences for bone health .
	manualset3
242073	4	423724	15	NULL	NULL	0	NULL	lactation 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As not many studies with phytase have been performed during gestation and lactation in sows yet , we can recommend , that phytase as supplement can be used to keep P in the diet at a lower level without negative consequences for bone health .
	manualset3
242075	5	423724	15	NULL	NULL	0	NULL	sows	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	As not many studies with phytase have been performed during gestation and lactation in sows yet , we can recommend , that phytase as supplement can be used to keep P in the diet at a lower level without negative consequences for bone health .
	manualset3
242079	6	423724	15	NULL	NULL	NULL	NULL	phytase as supplement	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As not many studies with phytase have been performed during gestation and lactation in sows yet , we can recommend , that phytase as supplement can be used to keep P in the diet at a lower level without negative consequences for bone health .
	manualset3
242082	7	423724	15	NULL	NULL	0	NULL	P	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	As not many studies with phytase have been performed during gestation and lactation in sows yet , we can recommend , that phytase as supplement can be used to keep P in the diet at a lower level without negative consequences for bone health .
	manualset3
242083	8	423724	15	NULL	NULL	0	NULL	diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	As not many studies with phytase have been performed during gestation and lactation in sows yet , we can recommend , that phytase as supplement can be used to keep P in the diet at a lower level without negative consequences for bone health .
	manualset3
242084	9	423724	15	NULL	NULL	0	NULL	level 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As not many studies with phytase have been performed during gestation and lactation in sows yet , we can recommend , that phytase as supplement can be used to keep P in the diet at a lower level without negative consequences for bone health .
	manualset3
242085	10	423724	15	NULL	NULL	0	NULL	negative consequences for bone health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As not many studies with phytase have been performed during gestation and lactation in sows yet , we can recommend , that phytase as supplement can be used to keep P in the diet at a lower level without negative consequences for bone health .
	manualset3
242086	1	423725	15	NULL	NULL	0	NULL	effective date	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	As of the effective date of this regulation , we will replace the DRB step with review by the Appeals Council .
	manualset3
242087	2	423725	15	NULL	NULL	0	NULL	regulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As of the effective date of this regulation , we will replace the DRB step with review by the Appeals Council .
	manualset3
242088	3	423725	15	NULL	NULL	NULL	NULL	DRB step	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As of the effective date of this regulation , we will replace the DRB step with review by the Appeals Council .
	manualset3
242089	4	423725	15	NULL	NULL	0	NULL	review 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	As of the effective date of this regulation , we will replace the DRB step with review by the Appeals Council .
	manualset3
242090	5	423725	15	NULL	NULL	0	NULL	Appeals Council	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	As of the effective date of this regulation , we will replace the DRB step with review by the Appeals Council .
	manualset3
242091	1	423726	15	NULL	NULL	0	NULL	organ transplant surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As organ transplant surgery continues to grow , effective organ preservation techniques and technology will expand as well .
	manualset3
242092	2	423726	15	NULL	NULL	0	NULL	effective organ preservation techniques	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As organ transplant surgery continues to grow , effective organ preservation techniques and technology will expand as well .
	manualset3
242093	3	423726	15	NULL	NULL	0	NULL	effective organ preservation technology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As organ transplant surgery continues to grow , effective organ preservation techniques and technology will expand as well .
	manualset3
242094	1	423727	15	NULL	NULL	0	NULL	solution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As our solution , we present an automatic gain-controlled oscillator with two output signals , the oscillator frequency , and a signal that represents the damping of the quartz resonator .
	manualset3
242095	2	423727	15	NULL	NULL	0	NULL	automatic gain-controlled oscillator with two output signals	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	As our solution , we present an automatic gain-controlled oscillator with two output signals , the oscillator frequency , and a signal that represents the damping of the quartz resonator .
	manualset3
242096	3	423727	15	NULL	NULL	0	NULL	oscillator frequency	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As our solution , we present an automatic gain-controlled oscillator with two output signals , the oscillator frequency , and a signal that represents the damping of the quartz resonator .
	manualset3
242097	4	423727	15	NULL	NULL	0	NULL	signal	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As our solution , we present an automatic gain-controlled oscillator with two output signals , the oscillator frequency , and a signal that represents the damping of the quartz resonator .
	manualset3
242098	5	423727	15	NULL	NULL	0	NULL	damping of the quartz resonator	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As our solution , we present an automatic gain-controlled oscillator with two output signals , the oscillator frequency , and a signal that represents the damping of the quartz resonator .
	manualset3
242099	1	423728	15	NULL	NULL	0	NULL	part of a biracial pilot study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of a biracial pilot study of the ways black and white men manage the stresses of sexually acquired HIV infection , we have examined the relationship between social support and mental health and behaviors .
	manualset3
242100	2	423728	15	NULL	NULL	0	NULL	ways	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of a biracial pilot study of the ways black and white men manage the stresses of sexually acquired HIV infection , we have examined the relationship between social support and mental health and behaviors .
	manualset3
242101	3	423728	15	NULL	NULL	0	NULL	black men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of a biracial pilot study of the ways black and white men manage the stresses of sexually acquired HIV infection , we have examined the relationship between social support and mental health and behaviors .
	manualset3
242102	4	423728	15	NULL	NULL	0	NULL	white men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of a biracial pilot study of the ways black and white men manage the stresses of sexually acquired HIV infection , we have examined the relationship between social support and mental health and behaviors .
	manualset3
242103	5	423728	15	NULL	NULL	0	NULL	stresses of sexually acquired HIV infection 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of a biracial pilot study of the ways black and white men manage the stresses of sexually acquired HIV infection , we have examined the relationship between social support and mental health and behaviors .
	manualset3
242104	6	423728	15	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of a biracial pilot study of the ways black and white men manage the stresses of sexually acquired HIV infection , we have examined the relationship between social support and mental health and behaviors .
	manualset3
242105	7	423728	15	NULL	NULL	0	NULL	social support	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of a biracial pilot study of the ways black and white men manage the stresses of sexually acquired HIV infection , we have examined the relationship between social support and mental health and behaviors .
	manualset3
242106	8	423728	15	NULL	NULL	0	NULL	mental health	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of a biracial pilot study of the ways black and white men manage the stresses of sexually acquired HIV infection , we have examined the relationship between social support and mental health and behaviors .
	manualset3
242107	9	423728	15	NULL	NULL	0	NULL	behaviors	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of a biracial pilot study of the ways black and white men manage the stresses of sexually acquired HIV infection , we have examined the relationship between social support and mental health and behaviors .
	manualset3
242108	1	423729	15	NULL	NULL	0	NULL	part of a continuing study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of a continuing study of the development of the marsupial auditory system , auditory brainstem responses ( ABR ) were recorded and an ABR audiogram was constructed for five female Northern Quolls ( Dasyurus hallucatus ) , which are nocturnal carnivores .
	manualset3
242109	2	423729	15	NULL	NULL	0	NULL	development of the marsupial auditory system	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of a continuing study of the development of the marsupial auditory system , auditory brainstem responses ( ABR ) were recorded and an ABR audiogram was constructed for five female Northern Quolls ( Dasyurus hallucatus ) , which are nocturnal carnivores .
	manualset3
242110	3	423729	15	NULL	NULL	0	NULL	auditory brainstem responses ( ABR ) 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of a continuing study of the development of the marsupial auditory system , auditory brainstem responses ( ABR ) were recorded and an ABR audiogram was constructed for five female Northern Quolls ( Dasyurus hallucatus ) , which are nocturnal carnivores .
	manualset3
242111	4	423729	15	NULL	NULL	0	NULL	ABR audiogram	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of a continuing study of the development of the marsupial auditory system , auditory brainstem responses ( ABR ) were recorded and an ABR audiogram was constructed for five female Northern Quolls ( Dasyurus hallucatus ) , which are nocturnal carnivores .
	manualset3
242112	5	423729	15	NULL	NULL	0	NULL	five 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of a continuing study of the development of the marsupial auditory system , auditory brainstem responses ( ABR ) were recorded and an ABR audiogram was constructed for five female Northern Quolls ( Dasyurus hallucatus ) , which are nocturnal carnivores .
	manualset3
242113	6	423729	15	NULL	NULL	0	NULL	female Northern Quolls ( Dasyurus hallucatus ) 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of a continuing study of the development of the marsupial auditory system , auditory brainstem responses ( ABR ) were recorded and an ABR audiogram was constructed for five female Northern Quolls ( Dasyurus hallucatus ) , which are nocturnal carnivores .
	manualset3
242114	7	423729	15	NULL	NULL	0	NULL	nocturnal carnivores	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of a continuing study of the development of the marsupial auditory system , auditory brainstem responses ( ABR ) were recorded and an ABR audiogram was constructed for five female Northern Quolls ( Dasyurus hallucatus ) , which are nocturnal carnivores .
	manualset3
242115	1	423730	15	NULL	NULL	0	NULL	part of an assessment 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of an assessment of the ecology of AIV in Guatemala , we conducted active surveillance in wild birds on the Pacific and Atlantic coasts .
	manualset3
242116	2	423730	15	NULL	NULL	0	NULL	ecology of AIV	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of an assessment of the ecology of AIV in Guatemala , we conducted active surveillance in wild birds on the Pacific and Atlantic coasts .
	manualset3
242117	3	423730	15	NULL	NULL	0	NULL	Guatemala	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of an assessment of the ecology of AIV in Guatemala , we conducted active surveillance in wild birds on the Pacific and Atlantic coasts .
	manualset3
242118	4	423730	15	NULL	NULL	0	NULL	active surveillance	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of an assessment of the ecology of AIV in Guatemala , we conducted active surveillance in wild birds on the Pacific and Atlantic coasts .
	manualset3
242119	5	423730	15	NULL	NULL	0	NULL	wild birds	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of an assessment of the ecology of AIV in Guatemala , we conducted active surveillance in wild birds on the Pacific and Atlantic coasts .
	manualset3
242123	6	423730	15	NULL	NULL	0	NULL	Pacific coasts	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of an assessment of the ecology of AIV in Guatemala , we conducted active surveillance in wild birds on the Pacific and Atlantic coasts .
	manualset3
242124	7	423730	15	NULL	NULL	0	NULL	Atlantic coasts	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of an assessment of the ecology of AIV in Guatemala , we conducted active surveillance in wild birds on the Pacific and Atlantic coasts .
	manualset3
242125	1	423731	15	NULL	NULL	0	NULL	part of an ongoing scale development process	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of an ongoing scale development process , this study provides an initial examination of the psychometric properties and validity of a new interview-based negative symptom instrument , the Clinical Assessment Interview for Negative Symptoms ( CAINS ) , in outpatients with schizophrenia or schizoaffective disorder ( N = 37 ) .
	manualset3
242126	2	423731	15	NULL	NULL	0	NULL	study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of an ongoing scale development process , this study provides an initial examination of the psychometric properties and validity of a new interview-based negative symptom instrument , the Clinical Assessment Interview for Negative Symptoms ( CAINS ) , in outpatients with schizophrenia or schizoaffective disorder ( N = 37 ) .
	manualset3
242127	3	423731	15	NULL	NULL	NULL	NULL	initial examination	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As part of an ongoing scale development process , this study provides an initial examination of the psychometric properties and validity of a new interview-based negative symptom instrument , the Clinical Assessment Interview for Negative Symptoms ( CAINS ) , in outpatients with schizophrenia or schizoaffective disorder ( N = 37 ) .
	manualset3
242128	4	423731	15	NULL	NULL	0	NULL	psychometric properties 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of an ongoing scale development process , this study provides an initial examination of the psychometric properties and validity of a new interview-based negative symptom instrument , the Clinical Assessment Interview for Negative Symptoms ( CAINS ) , in outpatients with schizophrenia or schizoaffective disorder ( N = 37 ) .
	manualset3
242129	5	423731	15	NULL	NULL	0	NULL	validity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of an ongoing scale development process , this study provides an initial examination of the psychometric properties and validity of a new interview-based negative symptom instrument , the Clinical Assessment Interview for Negative Symptoms ( CAINS ) , in outpatients with schizophrenia or schizoaffective disorder ( N = 37 ) .
	manualset3
242130	6	423731	15	NULL	NULL	0	NULL	interview-based negative symptom instrument 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of an ongoing scale development process , this study provides an initial examination of the psychometric properties and validity of a new interview-based negative symptom instrument , the Clinical Assessment Interview for Negative Symptoms ( CAINS ) , in outpatients with schizophrenia or schizoaffective disorder ( N = 37 ) .
	manualset3
242131	7	423731	15	NULL	NULL	0	NULL	Clinical Assessment Interview 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of an ongoing scale development process , this study provides an initial examination of the psychometric properties and validity of a new interview-based negative symptom instrument , the Clinical Assessment Interview for Negative Symptoms ( CAINS ) , in outpatients with schizophrenia or schizoaffective disorder ( N = 37 ) .
	manualset3
242132	8	423731	15	NULL	NULL	0	NULL	Negative Symptoms ( CAINS )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of an ongoing scale development process , this study provides an initial examination of the psychometric properties and validity of a new interview-based negative symptom instrument , the Clinical Assessment Interview for Negative Symptoms ( CAINS ) , in outpatients with schizophrenia or schizoaffective disorder ( N = 37 ) .
	manualset3
242133	9	423731	15	NULL	NULL	0	NULL	outpatients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of an ongoing scale development process , this study provides an initial examination of the psychometric properties and validity of a new interview-based negative symptom instrument , the Clinical Assessment Interview for Negative Symptoms ( CAINS ) , in outpatients with schizophrenia or schizoaffective disorder ( N = 37 ) .
	manualset3
242134	10	423731	15	NULL	NULL	0	NULL	schizophrenia 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of an ongoing scale development process , this study provides an initial examination of the psychometric properties and validity of a new interview-based negative symptom instrument , the Clinical Assessment Interview for Negative Symptoms ( CAINS ) , in outpatients with schizophrenia or schizoaffective disorder ( N = 37 ) .
	manualset3
242135	11	423731	15	NULL	NULL	0	NULL	schizoaffective disorder 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of an ongoing scale development process , this study provides an initial examination of the psychometric properties and validity of a new interview-based negative symptom instrument , the Clinical Assessment Interview for Negative Symptoms ( CAINS ) , in outpatients with schizophrenia or schizoaffective disorder ( N = 37 ) .
	manualset3
242136	12	423731	15	NULL	NULL	0	NULL	N = 37	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of an ongoing scale development process , this study provides an initial examination of the psychometric properties and validity of a new interview-based negative symptom instrument , the Clinical Assessment Interview for Negative Symptoms ( CAINS ) , in outpatients with schizophrenia or schizoaffective disorder ( N = 37 ) .
	manualset3
242142	1	423732	15	NULL	NULL	0	NULL	Effects of 6-methyl-uracil	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of 6-methyl-uracil upon the phagocytic activity in mice following whole-body X-irradiation OR 2 , 4 , 6-triethyleneimino-s-triazine treatment ( author 's transl ) ) .
	manualset3
242143	2	423732	15	NULL	NULL	0	NULL	phagocytic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of 6-methyl-uracil upon the phagocytic activity in mice following whole-body X-irradiation OR 2 , 4 , 6-triethyleneimino-s-triazine treatment ( author 's transl ) ) .
	manualset3
242144	3	423732	15	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of 6-methyl-uracil upon the phagocytic activity in mice following whole-body X-irradiation OR 2 , 4 , 6-triethyleneimino-s-triazine treatment ( author 's transl ) ) .
	manualset3
242145	4	423732	15	NULL	NULL	NULL	NULL	whole-body X-irradiation 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Effects of 6-methyl-uracil upon the phagocytic activity in mice following whole-body X-irradiation OR 2 , 4 , 6-triethyleneimino-s-triazine treatment ( author 's transl ) ) .
	manualset3
242147	5	423732	15	NULL	NULL	NULL	NULL	2 , 4 , 6-triethyleneimino-s-triazine treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Effects of 6-methyl-uracil upon the phagocytic activity in mice following whole-body X-irradiation OR 2 , 4 , 6-triethyleneimino-s-triazine treatment ( author 's transl ) ) .
	manualset3
242937	6	423732	15	NULL	NULL	NULL	NULL	author 's transl	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Effects of 6-methyl-uracil upon the phagocytic activity in mice following whole-body X-irradiation OR 2 , 4 , 6-triethyleneimino-s-triazine treatment ( author 's transl ) ) .
	manualset3
242149	1	423733	15	NULL	NULL	0	NULL	part of the temperature effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of the temperature effects study on the sorption of metallic cations onto zirconium diphosphate , we have first investigated the intrinsic surface properties of this synthetic compound for different temperatures ( 25 , 50 , 75 and 90 degrees C ) .
	manualset3
242150	2	423733	15	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of the temperature effects study on the sorption of metallic cations onto zirconium diphosphate , we have first investigated the intrinsic surface properties of this synthetic compound for different temperatures ( 25 , 50 , 75 and 90 degrees C ) .
	manualset3
242151	3	423733	15	NULL	NULL	0	NULL	sorption of metallic cations onto zirconium diphosphate	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of the temperature effects study on the sorption of metallic cations onto zirconium diphosphate , we have first investigated the intrinsic surface properties of this synthetic compound for different temperatures ( 25 , 50 , 75 and 90 degrees C ) .
	manualset3
242155	4	423733	15	NULL	NULL	0	NULL	intrinsic surface properties	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of the temperature effects study on the sorption of metallic cations onto zirconium diphosphate , we have first investigated the intrinsic surface properties of this synthetic compound for different temperatures ( 25 , 50 , 75 and 90 degrees C ) .
	manualset3
242170	5	423733	15	NULL	NULL	0	NULL	 synthetic compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of the temperature effects study on the sorption of metallic cations onto zirconium diphosphate , we have first investigated the intrinsic surface properties of this synthetic compound for different temperatures ( 25 , 50 , 75 and 90 degrees C ) .
	manualset3
242171	6	423733	15	NULL	NULL	0	NULL	temperatures	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of the temperature effects study on the sorption of metallic cations onto zirconium diphosphate , we have first investigated the intrinsic surface properties of this synthetic compound for different temperatures ( 25 , 50 , 75 and 90 degrees C ) .
	manualset3
242172	7	423733	15	NULL	NULL	0	NULL	25 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of the temperature effects study on the sorption of metallic cations onto zirconium diphosphate , we have first investigated the intrinsic surface properties of this synthetic compound for different temperatures ( 25 , 50 , 75 and 90 degrees C ) .
	manualset3
242173	8	423733	15	NULL	NULL	0	NULL	50 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of the temperature effects study on the sorption of metallic cations onto zirconium diphosphate , we have first investigated the intrinsic surface properties of this synthetic compound for different temperatures ( 25 , 50 , 75 and 90 degrees C ) .
	manualset3
242174	9	423733	15	NULL	NULL	0	NULL	75 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of the temperature effects study on the sorption of metallic cations onto zirconium diphosphate , we have first investigated the intrinsic surface properties of this synthetic compound for different temperatures ( 25 , 50 , 75 and 90 degrees C ) .
	manualset3
242175	10	423733	15	NULL	NULL	0	NULL	90 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of the temperature effects study on the sorption of metallic cations onto zirconium diphosphate , we have first investigated the intrinsic surface properties of this synthetic compound for different temperatures ( 25 , 50 , 75 and 90 degrees C ) .
	manualset3
242176	1	423734	15	NULL	NULL	0	NULL	 part of this strategy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of this strategy we have constructed a high-resolution genetic map of the chromosome segment surrounding Gro1 , based on RFLP , RAPD and AFLP markers .
	manualset3
242177	2	423734	15	NULL	NULL	0	NULL	high-resolution genetic map	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of this strategy we have constructed a high-resolution genetic map of the chromosome segment surrounding Gro1 , based on RFLP , RAPD and AFLP markers .
	manualset3
242178	3	423734	15	NULL	NULL	0	NULL	chromosome segment surrounding Gro1	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of this strategy we have constructed a high-resolution genetic map of the chromosome segment surrounding Gro1 , based on RFLP , RAPD and AFLP markers .
	manualset3
242179	4	423734	15	NULL	NULL	NULL	NULL	RFLP markers	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As part of this strategy we have constructed a high-resolution genetic map of the chromosome segment surrounding Gro1 , based on RFLP , RAPD and AFLP markers .
	manualset3
242180	5	423734	15	NULL	NULL	0	NULL	RAPD markers	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of this strategy we have constructed a high-resolution genetic map of the chromosome segment surrounding Gro1 , based on RFLP , RAPD and AFLP markers .
	manualset3
242181	6	423734	15	NULL	NULL	0	NULL	AFLP markers	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	As part of this strategy we have constructed a high-resolution genetic map of the chromosome segment surrounding Gro1 , based on RFLP , RAPD and AFLP markers .
	manualset3
242182	1	423735	15	NULL	NULL	0	NULL	precipitation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As precipitation of contaminating non-viral protein increases with increasing PEG concentrations , best results with respect to purity and recovery were obtained at 5 % PEG 6000 .
	manualset3
242183	2	423735	15	NULL	NULL	0	NULL	non-viral protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	As precipitation of contaminating non-viral protein increases with increasing PEG concentrations , best results with respect to purity and recovery were obtained at 5 % PEG 6000 .
	manualset3
242184	3	423735	15	NULL	NULL	0	NULL	PEG concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As precipitation of contaminating non-viral protein increases with increasing PEG concentrations , best results with respect to purity and recovery were obtained at 5 % PEG 6000 .
	manualset3
242185	4	423735	15	NULL	NULL	0	NULL	results	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As precipitation of contaminating non-viral protein increases with increasing PEG concentrations , best results with respect to purity and recovery were obtained at 5 % PEG 6000 .
	manualset3
242186	5	423735	15	NULL	NULL	0	NULL	purity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As precipitation of contaminating non-viral protein increases with increasing PEG concentrations , best results with respect to purity and recovery were obtained at 5 % PEG 6000 .
	manualset3
242187	6	423735	15	NULL	NULL	0	NULL	recovery	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As precipitation of contaminating non-viral protein increases with increasing PEG concentrations , best results with respect to purity and recovery were obtained at 5 % PEG 6000 .
	manualset3
242188	7	423735	15	NULL	NULL	0	NULL	5 % PEG 6000	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As precipitation of contaminating non-viral protein increases with increasing PEG concentrations , best results with respect to purity and recovery were obtained at 5 % PEG 6000 .
	manualset3
242189	1	423736	15	NULL	NULL	0	NULL	pregel concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As pregel concentration increased ( from 5 to 45 % for the rheometer and from 0 to 60 % for the extruder ) , the amount of water available in the system for gelatinization of existing raw starch granules decreased due to the stronger water-binding capacity of pregelatinized starch .
	manualset3
242190	2	423736	15	NULL	NULL	0	NULL	5 to 45 % for the rheometer	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As pregel concentration increased ( from 5 to 45 % for the rheometer and from 0 to 60 % for the extruder ) , the amount of water available in the system for gelatinization of existing raw starch granules decreased due to the stronger water-binding capacity of pregelatinized starch .
	manualset3
242191	3	423736	15	NULL	NULL	0	NULL	0 to 60 % for the extruder	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As pregel concentration increased ( from 5 to 45 % for the rheometer and from 0 to 60 % for the extruder ) , the amount of water available in the system for gelatinization of existing raw starch granules decreased due to the stronger water-binding capacity of pregelatinized starch .
	manualset3
242192	4	423736	15	NULL	NULL	0	NULL	amount of water 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As pregel concentration increased ( from 5 to 45 % for the rheometer and from 0 to 60 % for the extruder ) , the amount of water available in the system for gelatinization of existing raw starch granules decreased due to the stronger water-binding capacity of pregelatinized starch .
	manualset3
242193	5	423736	15	NULL	NULL	0	NULL	system for gelatinization 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As pregel concentration increased ( from 5 to 45 % for the rheometer and from 0 to 60 % for the extruder ) , the amount of water available in the system for gelatinization of existing raw starch granules decreased due to the stronger water-binding capacity of pregelatinized starch .
	manualset3
242194	6	423736	15	NULL	NULL	0	NULL	raw starch granules	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	As pregel concentration increased ( from 5 to 45 % for the rheometer and from 0 to 60 % for the extruder ) , the amount of water available in the system for gelatinization of existing raw starch granules decreased due to the stronger water-binding capacity of pregelatinized starch .
	manualset3
242195	7	423736	15	NULL	NULL	0	NULL	stronger water-binding capacity 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As pregel concentration increased ( from 5 to 45 % for the rheometer and from 0 to 60 % for the extruder ) , the amount of water available in the system for gelatinization of existing raw starch granules decreased due to the stronger water-binding capacity of pregelatinized starch .
	manualset3
242196	8	423736	15	NULL	NULL	0	NULL	pregelatinized starch	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	As pregel concentration increased ( from 5 to 45 % for the rheometer and from 0 to 60 % for the extruder ) , the amount of water available in the system for gelatinization of existing raw starch granules decreased due to the stronger water-binding capacity of pregelatinized starch .
	manualset3
242197	1	423737	15	NULL	NULL	NULL	NULL	preliminary validation of this approach	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As preliminary validation of this approach , short-term micro-tensile bond strengths to acid-etched and primed dentin were significantly enhanced by nanogel inclusion in the adhesive resins .
	manualset3
242198	2	423737	15	NULL	NULL	0	NULL	short-term micro-tensile bond strengths	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As preliminary validation of this approach , short-term micro-tensile bond strengths to acid-etched and primed dentin were significantly enhanced by nanogel inclusion in the adhesive resins .
	manualset3
242199	3	423737	15	NULL	NULL	0	NULL	acid-etched dentin	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As preliminary validation of this approach , short-term micro-tensile bond strengths to acid-etched and primed dentin were significantly enhanced by nanogel inclusion in the adhesive resins .
	manualset3
242200	4	423737	15	NULL	NULL	0	NULL	primed dentin 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As preliminary validation of this approach , short-term micro-tensile bond strengths to acid-etched and primed dentin were significantly enhanced by nanogel inclusion in the adhesive resins .
	manualset3
242201	5	423737	15	NULL	NULL	0	NULL	nanogel inclusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As preliminary validation of this approach , short-term micro-tensile bond strengths to acid-etched and primed dentin were significantly enhanced by nanogel inclusion in the adhesive resins .
	manualset3
242202	6	423737	15	NULL	NULL	0	NULL	adhesive resins	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	As preliminary validation of this approach , short-term micro-tensile bond strengths to acid-etched and primed dentin were significantly enhanced by nanogel inclusion in the adhesive resins .
	manualset3
242256	1	423738	15	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As presence of CIS is asymptomatic , a simple screening method is needed when CIS is suspected ( i.e. in males investigated for infertility ) .
	manualset3
242257	2	423738	15	NULL	NULL	0	NULL	CIS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As presence of CIS is asymptomatic , a simple screening method is needed when CIS is suspected ( i.e. in males investigated for infertility ) .
	manualset3
242258	3	423738	15	NULL	NULL	0	NULL	simple screening method	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As presence of CIS is asymptomatic , a simple screening method is needed when CIS is suspected ( i.e. in males investigated for infertility ) .
	manualset3
242259	4	423738	15	NULL	NULL	0	NULL	CIS 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As presence of CIS is asymptomatic , a simple screening method is needed when CIS is suspected ( i.e. in males investigated for infertility ) .
	manualset3
242260	5	423738	15	NULL	NULL	0	NULL	males	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As presence of CIS is asymptomatic , a simple screening method is needed when CIS is suspected ( i.e. in males investigated for infertility ) .
	manualset3
242261	6	423738	15	NULL	NULL	0	NULL	infertility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As presence of CIS is asymptomatic , a simple screening method is needed when CIS is suspected ( i.e. in males investigated for infertility ) .
	manualset3
242262	1	423739	15	NULL	NULL	0	NULL	US patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As previously reported , in US patients with acute KD , IgA plasma cells ( PCs ) infiltrate the vascular wall .
	manualset3
242266	2	423739	15	NULL	NULL	0	NULL	acute KD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	As previously reported , in US patients with acute KD , IgA plasma cells ( PCs ) infiltrate the vascular wall .
	manualset3
242270	3	423739	15	NULL	NULL	NULL	NULL	IgA plasma cells ( PCs )	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As previously reported , in US patients with acute KD , IgA plasma cells ( PCs ) infiltrate the vascular wall .
	manualset3
242271	4	423739	15	NULL	NULL	0	NULL	vascular wall	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	As previously reported , in US patients with acute KD , IgA plasma cells ( PCs ) infiltrate the vascular wall .
	manualset3
242278	1	423740	15	NULL	NULL	NULL	NULL	problems related to organ motion 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As problems related to organ motion are increasingly addressed , the use of IMRT in the treatment of lung cancer , particularly in non-small cell lung cancer and mesothelioma , continues to rise .
	manualset3
242279	2	423740	15	NULL	NULL	0	NULL	use of IMRT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As problems related to organ motion are increasingly addressed , the use of IMRT in the treatment of lung cancer , particularly in non-small cell lung cancer and mesothelioma , continues to rise .
	manualset3
242280	3	423740	15	NULL	NULL	0	NULL	treatment of lung cancer	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As problems related to organ motion are increasingly addressed , the use of IMRT in the treatment of lung cancer , particularly in non-small cell lung cancer and mesothelioma , continues to rise .
	manualset3
242281	4	423740	15	NULL	NULL	0	NULL	non-small cell lung cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	As problems related to organ motion are increasingly addressed , the use of IMRT in the treatment of lung cancer , particularly in non-small cell lung cancer and mesothelioma , continues to rise .
	manualset3
242282	5	423740	15	NULL	NULL	0	NULL	mesothelioma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	As problems related to organ motion are increasingly addressed , the use of IMRT in the treatment of lung cancer , particularly in non-small cell lung cancer and mesothelioma , continues to rise .
	manualset3
242286	1	423741	15	NULL	NULL	0	NULL	Effects of combined therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of combined therapy of Phosphatidylinositol 3p-Kinase and Paclitaxel in human lung cancer nude mice model . ) .
	manualset3
242287	2	423741	15	NULL	NULL	0	NULL	Phosphatidylinositol 3p-Kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of combined therapy of Phosphatidylinositol 3p-Kinase and Paclitaxel in human lung cancer nude mice model . ) .
	manualset3
242288	3	423741	15	NULL	NULL	0	NULL	Paclitaxel	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of combined therapy of Phosphatidylinositol 3p-Kinase and Paclitaxel in human lung cancer nude mice model . ) .
	manualset3
242289	4	423741	15	NULL	NULL	0	NULL	human lung cancer nude mice model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of combined therapy of Phosphatidylinositol 3p-Kinase and Paclitaxel in human lung cancer nude mice model . ) .
	manualset3
242295	1	423742	15	NULL	NULL	0	NULL	cytotoxic activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As regards the cytotoxic activity of methylating agents ( N-methylnitrosourea , N-methyl-N ' - nitro-N-nitrosoguanidine , dimethylsulfate and temozolomide ) and other alkylators with different structure and different interactions with DNA such as CC-1065 and FCE-24517 ( minor groove binders known to bind to N3 of adenine ) , 4 - ( bis ( 2-chloroethyl ) amino ) - L-phenylalanine and cis-diamminedichloroplatinum II , cytotoxicity was the same for tag-expressing and non-expressing cells .
	manualset3
242298	2	423742	15	NULL	NULL	0	NULL	methylating agents 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	As regards the cytotoxic activity of methylating agents ( N-methylnitrosourea , N-methyl-N ' - nitro-N-nitrosoguanidine , dimethylsulfate and temozolomide ) and other alkylators with different structure and different interactions with DNA such as CC-1065 and FCE-24517 ( minor groove binders known to bind to N3 of adenine ) , 4 - ( bis ( 2-chloroethyl ) amino ) - L-phenylalanine and cis-diamminedichloroplatinum II , cytotoxicity was the same for tag-expressing and non-expressing cells .
	manualset3
242301	3	423742	15	NULL	NULL	NULL	NULL	N-methylnitrosourea	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As regards the cytotoxic activity of methylating agents ( N-methylnitrosourea , N-methyl-N ' - nitro-N-nitrosoguanidine , dimethylsulfate and temozolomide ) and other alkylators with different structure and different interactions with DNA such as CC-1065 and FCE-24517 ( minor groove binders known to bind to N3 of adenine ) , 4 - ( bis ( 2-chloroethyl ) amino ) - L-phenylalanine and cis-diamminedichloroplatinum II , cytotoxicity was the same for tag-expressing and non-expressing cells .
	manualset3
242304	5	423742	15	NULL	NULL	NULL	NULL	dimethylsulfate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As regards the cytotoxic activity of methylating agents ( N-methylnitrosourea , N-methyl-N ' - nitro-N-nitrosoguanidine , dimethylsulfate and temozolomide ) and other alkylators with different structure and different interactions with DNA such as CC-1065 and FCE-24517 ( minor groove binders known to bind to N3 of adenine ) , 4 - ( bis ( 2-chloroethyl ) amino ) - L-phenylalanine and cis-diamminedichloroplatinum II , cytotoxicity was the same for tag-expressing and non-expressing cells .
	manualset3
242305	7	423742	15	NULL	NULL	NULL	NULL	alkylators 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As regards the cytotoxic activity of methylating agents ( N-methylnitrosourea , N-methyl-N ' - nitro-N-nitrosoguanidine , dimethylsulfate and temozolomide ) and other alkylators with different structure and different interactions with DNA such as CC-1065 and FCE-24517 ( minor groove binders known to bind to N3 of adenine ) , 4 - ( bis ( 2-chloroethyl ) amino ) - L-phenylalanine and cis-diamminedichloroplatinum II , cytotoxicity was the same for tag-expressing and non-expressing cells .
	manualset3
242306	8	423742	15	NULL	NULL	NULL	NULL	 structure	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As regards the cytotoxic activity of methylating agents ( N-methylnitrosourea , N-methyl-N ' - nitro-N-nitrosoguanidine , dimethylsulfate and temozolomide ) and other alkylators with different structure and different interactions with DNA such as CC-1065 and FCE-24517 ( minor groove binders known to bind to N3 of adenine ) , 4 - ( bis ( 2-chloroethyl ) amino ) - L-phenylalanine and cis-diamminedichloroplatinum II , cytotoxicity was the same for tag-expressing and non-expressing cells .
	manualset3
242308	9	423742	15	NULL	NULL	NULL	NULL	interactions with DNA	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As regards the cytotoxic activity of methylating agents ( N-methylnitrosourea , N-methyl-N ' - nitro-N-nitrosoguanidine , dimethylsulfate and temozolomide ) and other alkylators with different structure and different interactions with DNA such as CC-1065 and FCE-24517 ( minor groove binders known to bind to N3 of adenine ) , 4 - ( bis ( 2-chloroethyl ) amino ) - L-phenylalanine and cis-diamminedichloroplatinum II , cytotoxicity was the same for tag-expressing and non-expressing cells .
	manualset3
242315	10	423742	15	NULL	NULL	NULL	NULL	CC-1065	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As regards the cytotoxic activity of methylating agents ( N-methylnitrosourea , N-methyl-N ' - nitro-N-nitrosoguanidine , dimethylsulfate and temozolomide ) and other alkylators with different structure and different interactions with DNA such as CC-1065 and FCE-24517 ( minor groove binders known to bind to N3 of adenine ) , 4 - ( bis ( 2-chloroethyl ) amino ) - L-phenylalanine and cis-diamminedichloroplatinum II , cytotoxicity was the same for tag-expressing and non-expressing cells .
	manualset3
242316	11	423742	15	NULL	NULL	NULL	NULL	FCE-24517	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As regards the cytotoxic activity of methylating agents ( N-methylnitrosourea , N-methyl-N ' - nitro-N-nitrosoguanidine , dimethylsulfate and temozolomide ) and other alkylators with different structure and different interactions with DNA such as CC-1065 and FCE-24517 ( minor groove binders known to bind to N3 of adenine ) , 4 - ( bis ( 2-chloroethyl ) amino ) - L-phenylalanine and cis-diamminedichloroplatinum II , cytotoxicity was the same for tag-expressing and non-expressing cells .
	manualset3
242320	12	423742	15	NULL	NULL	NULL	NULL	minor groove binders	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As regards the cytotoxic activity of methylating agents ( N-methylnitrosourea , N-methyl-N ' - nitro-N-nitrosoguanidine , dimethylsulfate and temozolomide ) and other alkylators with different structure and different interactions with DNA such as CC-1065 and FCE-24517 ( minor groove binders known to bind to N3 of adenine ) , 4 - ( bis ( 2-chloroethyl ) amino ) - L-phenylalanine and cis-diamminedichloroplatinum II , cytotoxicity was the same for tag-expressing and non-expressing cells .
	manualset3
242324	13	423742	15	NULL	NULL	NULL	NULL	N3 of adenine	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As regards the cytotoxic activity of methylating agents ( N-methylnitrosourea , N-methyl-N ' - nitro-N-nitrosoguanidine , dimethylsulfate and temozolomide ) and other alkylators with different structure and different interactions with DNA such as CC-1065 and FCE-24517 ( minor groove binders known to bind to N3 of adenine ) , 4 - ( bis ( 2-chloroethyl ) amino ) - L-phenylalanine and cis-diamminedichloroplatinum II , cytotoxicity was the same for tag-expressing and non-expressing cells .
	manualset3
242325	14	423742	15	NULL	NULL	NULL	NULL	4 - ( bis ( 2-chloroethyl ) amino ) - L-phenylalanine	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As regards the cytotoxic activity of methylating agents ( N-methylnitrosourea , N-methyl-N ' - nitro-N-nitrosoguanidine , dimethylsulfate and temozolomide ) and other alkylators with different structure and different interactions with DNA such as CC-1065 and FCE-24517 ( minor groove binders known to bind to N3 of adenine ) , 4 - ( bis ( 2-chloroethyl ) amino ) - L-phenylalanine and cis-diamminedichloroplatinum II , cytotoxicity was the same for tag-expressing and non-expressing cells .
	manualset3
242326	15	423742	15	NULL	NULL	NULL	NULL	cis-diamminedichloroplatinum II 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As regards the cytotoxic activity of methylating agents ( N-methylnitrosourea , N-methyl-N ' - nitro-N-nitrosoguanidine , dimethylsulfate and temozolomide ) and other alkylators with different structure and different interactions with DNA such as CC-1065 and FCE-24517 ( minor groove binders known to bind to N3 of adenine ) , 4 - ( bis ( 2-chloroethyl ) amino ) - L-phenylalanine and cis-diamminedichloroplatinum II , cytotoxicity was the same for tag-expressing and non-expressing cells .
	manualset3
242327	16	423742	15	NULL	NULL	NULL	NULL	cytotoxicity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As regards the cytotoxic activity of methylating agents ( N-methylnitrosourea , N-methyl-N ' - nitro-N-nitrosoguanidine , dimethylsulfate and temozolomide ) and other alkylators with different structure and different interactions with DNA such as CC-1065 and FCE-24517 ( minor groove binders known to bind to N3 of adenine ) , 4 - ( bis ( 2-chloroethyl ) amino ) - L-phenylalanine and cis-diamminedichloroplatinum II , cytotoxicity was the same for tag-expressing and non-expressing cells .
	manualset3
242329	17	423742	15	NULL	NULL	NULL	NULL	tag-expressing cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As regards the cytotoxic activity of methylating agents ( N-methylnitrosourea , N-methyl-N ' - nitro-N-nitrosoguanidine , dimethylsulfate and temozolomide ) and other alkylators with different structure and different interactions with DNA such as CC-1065 and FCE-24517 ( minor groove binders known to bind to N3 of adenine ) , 4 - ( bis ( 2-chloroethyl ) amino ) - L-phenylalanine and cis-diamminedichloroplatinum II , cytotoxicity was the same for tag-expressing and non-expressing cells .
	manualset3
242332	18	423742	15	NULL	NULL	NULL	NULL	non-expressing cells 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As regards the cytotoxic activity of methylating agents ( N-methylnitrosourea , N-methyl-N ' - nitro-N-nitrosoguanidine , dimethylsulfate and temozolomide ) and other alkylators with different structure and different interactions with DNA such as CC-1065 and FCE-24517 ( minor groove binders known to bind to N3 of adenine ) , 4 - ( bis ( 2-chloroethyl ) amino ) - L-phenylalanine and cis-diamminedichloroplatinum II , cytotoxicity was the same for tag-expressing and non-expressing cells .
	manualset3
242368	6	423742	15	NULL	NULL	NULL	NULL	temozolomide	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As regards the cytotoxic activity of methylating agents ( N-methylnitrosourea , N-methyl-N ' - nitro-N-nitrosoguanidine , dimethylsulfate and temozolomide ) and other alkylators with different structure and different interactions with DNA such as CC-1065 and FCE-24517 ( minor groove binders known to bind to N3 of adenine ) , 4 - ( bis ( 2-chloroethyl ) amino ) - L-phenylalanine and cis-diamminedichloroplatinum II , cytotoxicity was the same for tag-expressing and non-expressing cells .
	manualset3
242374	4	423742	15	NULL	NULL	0	NULL	N-methyl-N ' - nitro-N-nitrosoguanidine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	As regards the cytotoxic activity of methylating agents ( N-methylnitrosourea , N-methyl-N ' - nitro-N-nitrosoguanidine , dimethylsulfate and temozolomide ) and other alkylators with different structure and different interactions with DNA such as CC-1065 and FCE-24517 ( minor groove binders known to bind to N3 of adenine ) , 4 - ( bis ( 2-chloroethyl ) amino ) - L-phenylalanine and cis-diamminedichloroplatinum II , cytotoxicity was the same for tag-expressing and non-expressing cells .
	manualset3
242391	1	423743	15	NULL	NULL	0	NULL	studies of HIV disease	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	As studies of HIV disease after the introduction of HAART continue to become available , more thorough descriptions of treated patients with ocular opportunistic infections will include side-effects and toxicities of therapy .
	manualset3
242392	2	423743	15	NULL	NULL	0	NULL	introduction of HAART	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As studies of HIV disease after the introduction of HAART continue to become available , more thorough descriptions of treated patients with ocular opportunistic infections will include side-effects and toxicities of therapy .
	manualset3
242393	3	423743	15	NULL	NULL	NULL	NULL	descriptions	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As studies of HIV disease after the introduction of HAART continue to become available , more thorough descriptions of treated patients with ocular opportunistic infections will include side-effects and toxicities of therapy .
	manualset3
242394	4	423743	15	NULL	NULL	0	NULL	treated patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As studies of HIV disease after the introduction of HAART continue to become available , more thorough descriptions of treated patients with ocular opportunistic infections will include side-effects and toxicities of therapy .
	manualset3
242395	5	423743	15	NULL	NULL	0	NULL	ocular opportunistic infections 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As studies of HIV disease after the introduction of HAART continue to become available , more thorough descriptions of treated patients with ocular opportunistic infections will include side-effects and toxicities of therapy .
	manualset3
242396	6	423743	15	NULL	NULL	0	NULL	side-effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As studies of HIV disease after the introduction of HAART continue to become available , more thorough descriptions of treated patients with ocular opportunistic infections will include side-effects and toxicities of therapy .
	manualset3
242397	7	423743	15	NULL	NULL	0	NULL	toxicities of therapy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As studies of HIV disease after the introduction of HAART continue to become available , more thorough descriptions of treated patients with ocular opportunistic infections will include side-effects and toxicities of therapy .
	manualset3
242398	1	423744	15	NULL	NULL	0	NULL	articles 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	As the articles indicate , if we are to achieve any measure of success , we must build our efforts and strategies on a foundation that embraces and encourages an integrated response .
	manualset3
242399	2	423744	15	NULL	NULL	0	NULL	measure of success	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As the articles indicate , if we are to achieve any measure of success , we must build our efforts and strategies on a foundation that embraces and encourages an integrated response .
	manualset3
242400	3	423744	15	NULL	NULL	0	NULL	efforts 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As the articles indicate , if we are to achieve any measure of success , we must build our efforts and strategies on a foundation that embraces and encourages an integrated response .
	manualset3
242401	4	423744	15	NULL	NULL	NULL	NULL	strategies	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As the articles indicate , if we are to achieve any measure of success , we must build our efforts and strategies on a foundation that embraces and encourages an integrated response .
	manualset3
242402	5	423744	15	NULL	NULL	0	NULL	foundation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As the articles indicate , if we are to achieve any measure of success , we must build our efforts and strategies on a foundation that embraces and encourages an integrated response .
	manualset3
242403	6	423744	15	NULL	NULL	0	NULL	integrated response	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As the articles indicate , if we are to achieve any measure of success , we must build our efforts and strategies on a foundation that embraces and encourages an integrated response .
	manualset3
242409	1	423745	15	NULL	NULL	0	NULL	culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	As the culture ages in vitro , however , changes appear in the morphology of the TIL along with degenerative changes and eventually death of the tumor cells .
	manualset3
242410	2	423745	15	NULL	NULL	0	NULL	changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As the culture ages in vitro , however , changes appear in the morphology of the TIL along with degenerative changes and eventually death of the tumor cells .
	manualset3
242411	3	423745	15	NULL	NULL	0	NULL	morphology of the TIL	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As the culture ages in vitro , however , changes appear in the morphology of the TIL along with degenerative changes and eventually death of the tumor cells .
	manualset3
242412	4	423745	15	NULL	NULL	0	NULL	degenerative changes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As the culture ages in vitro , however , changes appear in the morphology of the TIL along with degenerative changes and eventually death of the tumor cells .
	manualset3
242413	5	423745	15	NULL	NULL	0	NULL	death of the tumor cells 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As the culture ages in vitro , however , changes appear in the morphology of the TIL along with degenerative changes and eventually death of the tumor cells .
	manualset3
242415	1	423746	15	NULL	NULL	0	NULL	 fiber toxicity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As the fiber toxicity is catalyzed by iron ions in specific crystallographic sites and the mechanical behavior of synthetic chrysotile nanotubes is strongly affected by the iron doping extent , the characterization of Fe substitution to Mg and/or Si sites in the chrysotile structure appears highly important .
	manualset3
242417	2	423746	15	NULL	NULL	0	NULL	iron ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	As the fiber toxicity is catalyzed by iron ions in specific crystallographic sites and the mechanical behavior of synthetic chrysotile nanotubes is strongly affected by the iron doping extent , the characterization of Fe substitution to Mg and/or Si sites in the chrysotile structure appears highly important .
	manualset3
242420	3	423746	15	NULL	NULL	0	NULL	specific crystallographic sites	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As the fiber toxicity is catalyzed by iron ions in specific crystallographic sites and the mechanical behavior of synthetic chrysotile nanotubes is strongly affected by the iron doping extent , the characterization of Fe substitution to Mg and/or Si sites in the chrysotile structure appears highly important .
	manualset3
242422	4	423746	15	NULL	NULL	0	NULL	mechanical behavior of synthetic chrysotile nanotubes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As the fiber toxicity is catalyzed by iron ions in specific crystallographic sites and the mechanical behavior of synthetic chrysotile nanotubes is strongly affected by the iron doping extent , the characterization of Fe substitution to Mg and/or Si sites in the chrysotile structure appears highly important .
	manualset3
242425	5	423746	15	NULL	NULL	0	NULL	iron doping extent	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As the fiber toxicity is catalyzed by iron ions in specific crystallographic sites and the mechanical behavior of synthetic chrysotile nanotubes is strongly affected by the iron doping extent , the characterization of Fe substitution to Mg and/or Si sites in the chrysotile structure appears highly important .
	manualset3
242426	6	423746	15	NULL	NULL	0	NULL	characterization of Fe substitution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As the fiber toxicity is catalyzed by iron ions in specific crystallographic sites and the mechanical behavior of synthetic chrysotile nanotubes is strongly affected by the iron doping extent , the characterization of Fe substitution to Mg and/or Si sites in the chrysotile structure appears highly important .
	manualset3
242427	7	423746	15	NULL	NULL	0	NULL	Mg and/or Si sites	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As the fiber toxicity is catalyzed by iron ions in specific crystallographic sites and the mechanical behavior of synthetic chrysotile nanotubes is strongly affected by the iron doping extent , the characterization of Fe substitution to Mg and/or Si sites in the chrysotile structure appears highly important .
	manualset3
242428	8	423746	15	NULL	NULL	0	NULL	chrysotile structure	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As the fiber toxicity is catalyzed by iron ions in specific crystallographic sites and the mechanical behavior of synthetic chrysotile nanotubes is strongly affected by the iron doping extent , the characterization of Fe substitution to Mg and/or Si sites in the chrysotile structure appears highly important .
	manualset3
242429	1	423747	15	NULL	NULL	0	NULL	2 articles	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	As the first of 2 articles , this paper describes the problem of noncompliance in medical practice and reviews literature addressing compliance specific to headache management .
	manualset3
242430	2	423747	15	NULL	NULL	0	NULL	paper 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	As the first of 2 articles , this paper describes the problem of noncompliance in medical practice and reviews literature addressing compliance specific to headache management .
	manualset3
242431	3	423747	15	NULL	NULL	0	NULL	problem of noncompliance 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As the first of 2 articles , this paper describes the problem of noncompliance in medical practice and reviews literature addressing compliance specific to headache management .
	manualset3
242434	4	423747	15	NULL	NULL	0	NULL	medical practice	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As the first of 2 articles , this paper describes the problem of noncompliance in medical practice and reviews literature addressing compliance specific to headache management .
	manualset3
242435	5	423747	15	NULL	NULL	0	NULL	reviews literature	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	As the first of 2 articles , this paper describes the problem of noncompliance in medical practice and reviews literature addressing compliance specific to headache management .
	manualset3
242436	6	423747	15	NULL	NULL	0	NULL	compliance	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As the first of 2 articles , this paper describes the problem of noncompliance in medical practice and reviews literature addressing compliance specific to headache management .
	manualset3
242437	7	423747	15	NULL	NULL	0	NULL	headache management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As the first of 2 articles , this paper describes the problem of noncompliance in medical practice and reviews literature addressing compliance specific to headache management .
	manualset3
242443	1	423748	15	NULL	NULL	0	NULL	importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As the importance of neurohormonal changes in the pathogenesis of worsening CHF is elucidated , newer medications aimed at counteracting such changes are becoming more important in the medical therapy of CHF in children .
	manualset3
242446	2	423748	15	NULL	NULL	0	NULL	neurohormonal changes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As the importance of neurohormonal changes in the pathogenesis of worsening CHF is elucidated , newer medications aimed at counteracting such changes are becoming more important in the medical therapy of CHF in children .
	manualset3
242447	3	423748	15	NULL	NULL	0	NULL	pathogenesis of worsening CHF 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As the importance of neurohormonal changes in the pathogenesis of worsening CHF is elucidated , newer medications aimed at counteracting such changes are becoming more important in the medical therapy of CHF in children .
	manualset3
242448	4	423748	15	NULL	NULL	0	NULL	medications 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	As the importance of neurohormonal changes in the pathogenesis of worsening CHF is elucidated , newer medications aimed at counteracting such changes are becoming more important in the medical therapy of CHF in children .
	manualset3
242450	5	423748	15	NULL	NULL	0	NULL	changes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As the importance of neurohormonal changes in the pathogenesis of worsening CHF is elucidated , newer medications aimed at counteracting such changes are becoming more important in the medical therapy of CHF in children .
	manualset3
242453	6	423748	15	NULL	NULL	0	NULL	medical therapy of CHF	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As the importance of neurohormonal changes in the pathogenesis of worsening CHF is elucidated , newer medications aimed at counteracting such changes are becoming more important in the medical therapy of CHF in children .
	manualset3
242454	7	423748	15	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As the importance of neurohormonal changes in the pathogenesis of worsening CHF is elucidated , newer medications aimed at counteracting such changes are becoming more important in the medical therapy of CHF in children .
	manualset3
242457	1	423749	15	NULL	NULL	0	NULL	post dimensions	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As the post dimensions are comparable to or smaller than the laser wavelength , near-field effects and localized electromagnetic fields are present in their vicinity .
	manualset3
242458	2	423749	15	NULL	NULL	0	NULL	laser wavelength	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As the post dimensions are comparable to or smaller than the laser wavelength , near-field effects and localized electromagnetic fields are present in their vicinity .
	manualset3
242459	3	423749	15	NULL	NULL	0	NULL	near-field effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As the post dimensions are comparable to or smaller than the laser wavelength , near-field effects and localized electromagnetic fields are present in their vicinity .
	manualset3
242461	4	423749	15	NULL	NULL	0	NULL	electromagnetic fields	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As the post dimensions are comparable to or smaller than the laser wavelength , near-field effects and localized electromagnetic fields are present in their vicinity .
	manualset3
242465	5	423749	15	NULL	NULL	0	NULL	vicinity	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	As the post dimensions are comparable to or smaller than the laser wavelength , near-field effects and localized electromagnetic fields are present in their vicinity .
	manualset3
242510	1	423750	15	NULL	NULL	0	NULL	relevance of this activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As the relevance of this activity to in vivo function is unknown , we have taken advantage of the conserved nature of ARF to study its function in Saccharomyces cerevisiae .
	manualset3
242511	2	423750	15	NULL	NULL	0	NULL	function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As the relevance of this activity to in vivo function is unknown , we have taken advantage of the conserved nature of ARF to study its function in Saccharomyces cerevisiae .
	manualset3
242512	3	423750	15	NULL	NULL	0	NULL	advantage 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As the relevance of this activity to in vivo function is unknown , we have taken advantage of the conserved nature of ARF to study its function in Saccharomyces cerevisiae .
	manualset3
242513	4	423750	15	NULL	NULL	0	NULL	conserved nature of ARF	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As the relevance of this activity to in vivo function is unknown , we have taken advantage of the conserved nature of ARF to study its function in Saccharomyces cerevisiae .
	manualset3
242514	5	423750	15	NULL	NULL	0	NULL	function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As the relevance of this activity to in vivo function is unknown , we have taken advantage of the conserved nature of ARF to study its function in Saccharomyces cerevisiae .
	manualset3
242515	6	423750	15	NULL	NULL	0	NULL	Saccharomyces cerevisiae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	As the relevance of this activity to in vivo function is unknown , we have taken advantage of the conserved nature of ARF to study its function in Saccharomyces cerevisiae .
	manualset3
242518	1	423751	15	NULL	NULL	0	NULL	Effects of cyclosporine 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of cyclosporine and blood transfusion on cardiac xenografts in combination of rat and mouse ) .
	manualset3
242520	2	423751	15	NULL	NULL	NULL	NULL	blood transfusion	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Effects of cyclosporine and blood transfusion on cardiac xenografts in combination of rat and mouse ) .
	manualset3
242531	3	423751	15	NULL	NULL	0	NULL	cardiac xenografts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of cyclosporine and blood transfusion on cardiac xenografts in combination of rat and mouse ) .
	manualset3
242532	4	423751	15	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of cyclosporine and blood transfusion on cardiac xenografts in combination of rat and mouse ) .
	manualset3
242533	5	423751	15	NULL	NULL	0	NULL	rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of cyclosporine and blood transfusion on cardiac xenografts in combination of rat and mouse ) .
	manualset3
242534	6	423751	15	NULL	NULL	0	NULL	mouse 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of cyclosporine and blood transfusion on cardiac xenografts in combination of rat and mouse ) .
	manualset3
242535	1	423752	15	NULL	NULL	0	NULL	comparison 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	As the result of the comparison of C - and G-banding patterns , and compare with other species in the genus Niviventer , we suppose that the chromosomal evolution of Niviventer involved in pericentric inversion and heterochromatin growth .
	manualset3
242536	2	423752	15	NULL	NULL	0	NULL	C -banding patterns	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	As the result of the comparison of C - and G-banding patterns , and compare with other species in the genus Niviventer , we suppose that the chromosomal evolution of Niviventer involved in pericentric inversion and heterochromatin growth .
	manualset3
242537	3	423752	15	NULL	NULL	0	NULL	G-banding patterns	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	As the result of the comparison of C - and G-banding patterns , and compare with other species in the genus Niviventer , we suppose that the chromosomal evolution of Niviventer involved in pericentric inversion and heterochromatin growth .
	manualset3
242538	4	423752	15	NULL	NULL	0	NULL	species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	As the result of the comparison of C - and G-banding patterns , and compare with other species in the genus Niviventer , we suppose that the chromosomal evolution of Niviventer involved in pericentric inversion and heterochromatin growth .
	manualset3
242539	5	423752	15	NULL	NULL	0	NULL	genus Niviventer	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	As the result of the comparison of C - and G-banding patterns , and compare with other species in the genus Niviventer , we suppose that the chromosomal evolution of Niviventer involved in pericentric inversion and heterochromatin growth .
	manualset3
242540	6	423752	15	NULL	NULL	0	NULL	chromosomal evolution of Niviventer 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As the result of the comparison of C - and G-banding patterns , and compare with other species in the genus Niviventer , we suppose that the chromosomal evolution of Niviventer involved in pericentric inversion and heterochromatin growth .
	manualset3
242541	7	423752	15	NULL	NULL	0	NULL	pericentric inversion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As the result of the comparison of C - and G-banding patterns , and compare with other species in the genus Niviventer , we suppose that the chromosomal evolution of Niviventer involved in pericentric inversion and heterochromatin growth .
	manualset3
242542	8	423752	15	NULL	NULL	0	NULL	heterochromatin growth	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As the result of the comparison of C - and G-banding patterns , and compare with other species in the genus Niviventer , we suppose that the chromosomal evolution of Niviventer involved in pericentric inversion and heterochromatin growth .
	manualset3
242543	1	423753	15	NULL	NULL	0	NULL	use of cyclosporine	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As the use of cyclosporine in small animals is increasing , further work is required to substantiate and quantify the proposed increased risk .
	manualset3
242544	2	423753	15	NULL	NULL	0	NULL	small animals 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	As the use of cyclosporine in small animals is increasing , further work is required to substantiate and quantify the proposed increased risk .
	manualset3
242545	3	423753	15	NULL	NULL	0	NULL	work	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	As the use of cyclosporine in small animals is increasing , further work is required to substantiate and quantify the proposed increased risk .
	manualset3
242546	4	423753	15	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As the use of cyclosporine in small animals is increasing , further work is required to substantiate and quantify the proposed increased risk .
	manualset3
242547	1	423754	15	NULL	NULL	0	NULL	divergent/paradoxical results 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	As these divergent/paradoxical results of FK506 may at least in part be attributable to differences in FK506 dosing , we have , in the current study , assessed dose-dependent effects of FK506 on atherosclerotic lesion formation as well as on inflammatory parameters relevant to atherosclerosis .
	manualset3
242548	2	423754	15	NULL	NULL	0	NULL	FK506 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	As these divergent/paradoxical results of FK506 may at least in part be attributable to differences in FK506 dosing , we have , in the current study , assessed dose-dependent effects of FK506 on atherosclerotic lesion formation as well as on inflammatory parameters relevant to atherosclerosis .
	manualset3
242549	3	423754	15	NULL	NULL	0	NULL	part	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As these divergent/paradoxical results of FK506 may at least in part be attributable to differences in FK506 dosing , we have , in the current study , assessed dose-dependent effects of FK506 on atherosclerotic lesion formation as well as on inflammatory parameters relevant to atherosclerosis .
	manualset3
242550	4	423754	15	NULL	NULL	0	NULL	differences in FK506 dosing 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As these divergent/paradoxical results of FK506 may at least in part be attributable to differences in FK506 dosing , we have , in the current study , assessed dose-dependent effects of FK506 on atherosclerotic lesion formation as well as on inflammatory parameters relevant to atherosclerosis .
	manualset3
242551	5	423754	15	NULL	NULL	0	NULL	current study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	As these divergent/paradoxical results of FK506 may at least in part be attributable to differences in FK506 dosing , we have , in the current study , assessed dose-dependent effects of FK506 on atherosclerotic lesion formation as well as on inflammatory parameters relevant to atherosclerosis .
	manualset3
242552	6	423754	15	NULL	NULL	0	NULL	dose-dependent effects of FK506	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As these divergent/paradoxical results of FK506 may at least in part be attributable to differences in FK506 dosing , we have , in the current study , assessed dose-dependent effects of FK506 on atherosclerotic lesion formation as well as on inflammatory parameters relevant to atherosclerosis .
	manualset3
242553	7	423754	15	NULL	NULL	0	NULL	atherosclerotic lesion formation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As these divergent/paradoxical results of FK506 may at least in part be attributable to differences in FK506 dosing , we have , in the current study , assessed dose-dependent effects of FK506 on atherosclerotic lesion formation as well as on inflammatory parameters relevant to atherosclerosis .
	manualset3
242554	8	423754	15	NULL	NULL	0	NULL	inflammatory parameters	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As these divergent/paradoxical results of FK506 may at least in part be attributable to differences in FK506 dosing , we have , in the current study , assessed dose-dependent effects of FK506 on atherosclerotic lesion formation as well as on inflammatory parameters relevant to atherosclerosis .
	manualset3
242555	9	423754	15	NULL	NULL	0	NULL	atherosclerosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	As these divergent/paradoxical results of FK506 may at least in part be attributable to differences in FK506 dosing , we have , in the current study , assessed dose-dependent effects of FK506 on atherosclerotic lesion formation as well as on inflammatory parameters relevant to atherosclerosis .
	manualset3
242556	1	423755	15	NULL	NULL	0	NULL	findings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As these findings may be of importance when the Ki-67 labeling index is used as a criterion for tumor grading or for clinical prognostication , this necessitate identification of the antibody used in every case .
	manualset3
242557	2	423755	15	NULL	NULL	0	NULL	importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As these findings may be of importance when the Ki-67 labeling index is used as a criterion for tumor grading or for clinical prognostication , this necessitate identification of the antibody used in every case .
	manualset3
242558	3	423755	15	NULL	NULL	0	NULL	Ki-67 labeling index	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As these findings may be of importance when the Ki-67 labeling index is used as a criterion for tumor grading or for clinical prognostication , this necessitate identification of the antibody used in every case .
	manualset3
242559	4	423755	15	NULL	NULL	0	NULL	criterion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As these findings may be of importance when the Ki-67 labeling index is used as a criterion for tumor grading or for clinical prognostication , this necessitate identification of the antibody used in every case .
	manualset3
242560	5	423755	15	NULL	NULL	0	NULL	tumor grading 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As these findings may be of importance when the Ki-67 labeling index is used as a criterion for tumor grading or for clinical prognostication , this necessitate identification of the antibody used in every case .
	manualset3
242561	6	423755	15	NULL	NULL	0	NULL	clinical prognostication	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As these findings may be of importance when the Ki-67 labeling index is used as a criterion for tumor grading or for clinical prognostication , this necessitate identification of the antibody used in every case .
	manualset3
242562	7	423755	15	NULL	NULL	0	NULL	identification of the antibody	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As these findings may be of importance when the Ki-67 labeling index is used as a criterion for tumor grading or for clinical prognostication , this necessitate identification of the antibody used in every case .
	manualset3
242563	8	423755	15	NULL	NULL	0	NULL	case	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	As these findings may be of importance when the Ki-67 labeling index is used as a criterion for tumor grading or for clinical prognostication , this necessitate identification of the antibody used in every case .
	manualset3
242564	1	423756	15	NULL	NULL	0	NULL	reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As this reaction is close to equilibrium in the body and is pH dependent , the ratio of the ( 13 ) C signal intensities from H ( 13 ) CO ( 3 ) ( - ) and ( 13 ) CO ( 2 ) , measured using MRS , can be used to calculate pH in vivo .
	manualset3
242565	2	423756	15	NULL	NULL	0	NULL	equilibrium in the body	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As this reaction is close to equilibrium in the body and is pH dependent , the ratio of the ( 13 ) C signal intensities from H ( 13 ) CO ( 3 ) ( - ) and ( 13 ) CO ( 2 ) , measured using MRS , can be used to calculate pH in vivo .
	manualset3
242566	3	423756	15	NULL	NULL	NULL	NULL	pH	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As this reaction is close to equilibrium in the body and is pH dependent , the ratio of the ( 13 ) C signal intensities from H ( 13 ) CO ( 3 ) ( - ) and ( 13 ) CO ( 2 ) , measured using MRS , can be used to calculate pH in vivo .
	manualset3
242567	4	423756	15	NULL	NULL	0	NULL	ratio of the ( 13 ) C signal intensities	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As this reaction is close to equilibrium in the body and is pH dependent , the ratio of the ( 13 ) C signal intensities from H ( 13 ) CO ( 3 ) ( - ) and ( 13 ) CO ( 2 ) , measured using MRS , can be used to calculate pH in vivo .
	manualset3
242568	5	423756	15	NULL	NULL	0	NULL	H ( 13 ) CO ( 3 ) ( - ) 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As this reaction is close to equilibrium in the body and is pH dependent , the ratio of the ( 13 ) C signal intensities from H ( 13 ) CO ( 3 ) ( - ) and ( 13 ) CO ( 2 ) , measured using MRS , can be used to calculate pH in vivo .
	manualset3
242569	6	423756	15	NULL	NULL	0	NULL	( 13 ) CO ( 2 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As this reaction is close to equilibrium in the body and is pH dependent , the ratio of the ( 13 ) C signal intensities from H ( 13 ) CO ( 3 ) ( - ) and ( 13 ) CO ( 2 ) , measured using MRS , can be used to calculate pH in vivo .
	manualset3
242570	7	423756	15	NULL	NULL	0	NULL	MRS 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	As this reaction is close to equilibrium in the body and is pH dependent , the ratio of the ( 13 ) C signal intensities from H ( 13 ) CO ( 3 ) ( - ) and ( 13 ) CO ( 2 ) , measured using MRS , can be used to calculate pH in vivo .
	manualset3
242571	8	423756	15	NULL	NULL	0	NULL	pH 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As this reaction is close to equilibrium in the body and is pH dependent , the ratio of the ( 13 ) C signal intensities from H ( 13 ) CO ( 3 ) ( - ) and ( 13 ) CO ( 2 ) , measured using MRS , can be used to calculate pH in vivo .
	manualset3
242572	1	423757	15	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As to when to institute a therapy , we simultaneously evaluated the use of a microfluorometer as a monitor of flap survival .
	manualset3
242573	2	423757	15	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As to when to institute a therapy , we simultaneously evaluated the use of a microfluorometer as a monitor of flap survival .
	manualset3
242574	3	423757	15	NULL	NULL	0	NULL	microfluorometer	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	As to when to institute a therapy , we simultaneously evaluated the use of a microfluorometer as a monitor of flap survival .
	manualset3
242575	4	423757	15	NULL	NULL	0	NULL	monitor of flap survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As to when to institute a therapy , we simultaneously evaluated the use of a microfluorometer as a monitor of flap survival .
	manualset3
242576	1	423758	15	NULL	NULL	0	NULL	translation products	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As translation products , two proteins , p27x-III and p21x-III , were detected in addition to p40x .
	manualset3
242577	2	423758	15	NULL	NULL	0	NULL	two proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As translation products , two proteins , p27x-III and p21x-III , were detected in addition to p40x .
	manualset3
242578	3	423758	15	NULL	NULL	0	NULL	p27x-III	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	As translation products , two proteins , p27x-III and p21x-III , were detected in addition to p40x .
	manualset3
242579	4	423758	15	NULL	NULL	0	NULL	p21x-III	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	As translation products , two proteins , p27x-III and p21x-III , were detected in addition to p40x .
	manualset3
242580	5	423758	15	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As translation products , two proteins , p27x-III and p21x-III , were detected in addition to p40x .
	manualset3
242581	6	423758	15	NULL	NULL	0	NULL	p40x	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	As translation products , two proteins , p27x-III and p21x-III , were detected in addition to p40x .
	manualset3
242582	1	423759	15	NULL	NULL	NULL	NULL	Effects of different severities of hypoxia-ischemia 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Effects of different severities of hypoxia-ischemia on brain injury in neonatal rats ) .
	manualset3
242583	2	423759	15	NULL	NULL	0	NULL	brain injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of different severities of hypoxia-ischemia on brain injury in neonatal rats ) .
	manualset3
242584	3	423759	15	NULL	NULL	0	NULL	neonatal rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of different severities of hypoxia-ischemia on brain injury in neonatal rats ) .
	manualset3
242585	1	423760	15	NULL	NULL	0	NULL	xerostomia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	As xerostomia has a significant effect on a person 's quality of life , a multifaceted approach to treating xerostomia is presented .
	manualset3
242586	2	423760	15	NULL	NULL	0	NULL	 effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As xerostomia has a significant effect on a person 's quality of life , a multifaceted approach to treating xerostomia is presented .
	manualset3
242587	3	423760	15	NULL	NULL	0	NULL	person 's quality of life	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As xerostomia has a significant effect on a person 's quality of life , a multifaceted approach to treating xerostomia is presented .
	manualset3
242588	4	423760	15	NULL	NULL	0	NULL	multifaceted approach	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As xerostomia has a significant effect on a person 's quality of life , a multifaceted approach to treating xerostomia is presented .
	manualset3
242589	5	423760	15	NULL	NULL	0	NULL	treating xerostomia 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As xerostomia has a significant effect on a person 's quality of life , a multifaceted approach to treating xerostomia is presented .
	manualset3
242775	1	423761	15	NULL	NULL	0	NULL	percentage of class I priority	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As well , the percentage of class I priority ( the highest safety priority ) problem reports/recalls for anaesthesia devices was 10.2 % compared with 4.9 % for non-anaesthesia devices ( P & lt ; 0.05 ) .
	manualset3
242776	2	423761	15	NULL	NULL	0	NULL	safety priority	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As well , the percentage of class I priority ( the highest safety priority ) problem reports/recalls for anaesthesia devices was 10.2 % compared with 4.9 % for non-anaesthesia devices ( P & lt ; 0.05 ) .
	manualset3
242778	3	423761	15	NULL	NULL	0	NULL	problem reports	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As well , the percentage of class I priority ( the highest safety priority ) problem reports/recalls for anaesthesia devices was 10.2 % compared with 4.9 % for non-anaesthesia devices ( P & lt ; 0.05 ) .
	manualset3
242780	4	423761	15	NULL	NULL	0	NULL	recalls 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As well , the percentage of class I priority ( the highest safety priority ) problem reports/recalls for anaesthesia devices was 10.2 % compared with 4.9 % for non-anaesthesia devices ( P & lt ; 0.05 ) .
	manualset3
242781	5	423761	15	NULL	NULL	0	NULL	anaesthesia devices 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	As well , the percentage of class I priority ( the highest safety priority ) problem reports/recalls for anaesthesia devices was 10.2 % compared with 4.9 % for non-anaesthesia devices ( P & lt ; 0.05 ) .
	manualset3
242782	6	423761	15	NULL	NULL	0	NULL	10.2 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As well , the percentage of class I priority ( the highest safety priority ) problem reports/recalls for anaesthesia devices was 10.2 % compared with 4.9 % for non-anaesthesia devices ( P & lt ; 0.05 ) .
	manualset3
242783	7	423761	15	NULL	NULL	0	NULL	4.9 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As well , the percentage of class I priority ( the highest safety priority ) problem reports/recalls for anaesthesia devices was 10.2 % compared with 4.9 % for non-anaesthesia devices ( P & lt ; 0.05 ) .
	manualset3
242784	8	423761	15	NULL	NULL	0	NULL	non-anaesthesia devices 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	As well , the percentage of class I priority ( the highest safety priority ) problem reports/recalls for anaesthesia devices was 10.2 % compared with 4.9 % for non-anaesthesia devices ( P & lt ; 0.05 ) .
	manualset3
242785	9	423761	15	NULL	NULL	0	NULL	P & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As well , the percentage of class I priority ( the highest safety priority ) problem reports/recalls for anaesthesia devices was 10.2 % compared with 4.9 % for non-anaesthesia devices ( P & lt ; 0.05 ) .
	manualset3
242789	1	423762	15	NULL	NULL	0	NULL	C57 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	As before , C57 mice showed higher levels of ethanol responding , compared with DBA mice .
	manualset3
242790	2	423762	15	NULL	NULL	0	NULL	levels of ethanol	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As before , C57 mice showed higher levels of ethanol responding , compared with DBA mice .
	manualset3
242792	3	423762	15	NULL	NULL	0	NULL	DBA mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	As before , C57 mice showed higher levels of ethanol responding , compared with DBA mice .
	manualset3
242797	1	423763	15	NULL	NULL	0	NULL	lack of activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As assessed by the lack of activity of symplastic marker enzymes , the extracellular washing fluid was free from intracellular contaminations .
	manualset3
242798	2	423763	15	NULL	NULL	0	NULL	symplastic marker enzymes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As assessed by the lack of activity of symplastic marker enzymes , the extracellular washing fluid was free from intracellular contaminations .
	manualset3
242799	3	423763	15	NULL	NULL	0	NULL	extracellular washing fluid 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	As assessed by the lack of activity of symplastic marker enzymes , the extracellular washing fluid was free from intracellular contaminations .
	manualset3
242800	4	423763	15	NULL	NULL	0	NULL	intracellular contaminations	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	As assessed by the lack of activity of symplastic marker enzymes , the extracellular washing fluid was free from intracellular contaminations .
	manualset3
242801	1	423764	15	NULL	NULL	0	NULL	collapsin-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	As demonstrated for collapsin-1 , CNS myelin-evoked growth cone collapse was accompanied by a reduction of rhodamine-phalloidin staining most prominent in the growth cone periphery , suggesting actin filament disassembly .
	manualset3
242802	2	423764	15	NULL	NULL	0	NULL	CNS myelin-evoked growth cone collapse 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As demonstrated for collapsin-1 , CNS myelin-evoked growth cone collapse was accompanied by a reduction of rhodamine-phalloidin staining most prominent in the growth cone periphery , suggesting actin filament disassembly .
	manualset3
242803	3	423764	15	NULL	NULL	0	NULL	reduction of rhodamine-phalloidin staining	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As demonstrated for collapsin-1 , CNS myelin-evoked growth cone collapse was accompanied by a reduction of rhodamine-phalloidin staining most prominent in the growth cone periphery , suggesting actin filament disassembly .
	manualset3
242804	4	423764	15	NULL	NULL	0	NULL	growth cone periphery	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As demonstrated for collapsin-1 , CNS myelin-evoked growth cone collapse was accompanied by a reduction of rhodamine-phalloidin staining most prominent in the growth cone periphery , suggesting actin filament disassembly .
	manualset3
242805	5	423764	15	NULL	NULL	0	NULL	actin filament disassembly	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As demonstrated for collapsin-1 , CNS myelin-evoked growth cone collapse was accompanied by a reduction of rhodamine-phalloidin staining most prominent in the growth cone periphery , suggesting actin filament disassembly .
	manualset3
242806	1	423765	15	NULL	NULL	0	NULL	discussion	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	As evidenced in the above discussion , contaminating the blood supply would require a highly sophisticated plan resulting in effects of rather limited ultimate scope , and would have to evade an extremely effective screening process already in full force .
	manualset3
242807	2	423765	15	NULL	NULL	0	NULL	contaminating the blood supply	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As evidenced in the above discussion , contaminating the blood supply would require a highly sophisticated plan resulting in effects of rather limited ultimate scope , and would have to evade an extremely effective screening process already in full force .
	manualset3
242808	3	423765	15	NULL	NULL	0	NULL	sophisticated plan 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	As evidenced in the above discussion , contaminating the blood supply would require a highly sophisticated plan resulting in effects of rather limited ultimate scope , and would have to evade an extremely effective screening process already in full force .
	manualset3
242809	4	423765	15	NULL	NULL	0	NULL	effects of rather limited ultimate scope	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As evidenced in the above discussion , contaminating the blood supply would require a highly sophisticated plan resulting in effects of rather limited ultimate scope , and would have to evade an extremely effective screening process already in full force .
	manualset3
242810	5	423765	15	NULL	NULL	0	NULL	effective screening process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As evidenced in the above discussion , contaminating the blood supply would require a highly sophisticated plan resulting in effects of rather limited ultimate scope , and would have to evade an extremely effective screening process already in full force .
	manualset3
242811	6	423765	15	NULL	NULL	0	NULL	force	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As evidenced in the above discussion , contaminating the blood supply would require a highly sophisticated plan resulting in effects of rather limited ultimate scope , and would have to evade an extremely effective screening process already in full force .
	manualset3
242812	1	423766	15	NULL	NULL	0	NULL	role of KCa3 .1 in HLMC migration 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As predicted from the role of KCa3 .1 in HLMC migration , adenosine abolished HLMC chemotaxis to asthmatic airway smooth muscle-conditioned medium .
	manualset3
242813	2	423766	15	NULL	NULL	0	NULL	adenosine	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	As predicted from the role of KCa3 .1 in HLMC migration , adenosine abolished HLMC chemotaxis to asthmatic airway smooth muscle-conditioned medium .
	manualset3
242814	3	423766	15	NULL	NULL	0	NULL	HLMC chemotaxis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As predicted from the role of KCa3 .1 in HLMC migration , adenosine abolished HLMC chemotaxis to asthmatic airway smooth muscle-conditioned medium .
	manualset3
242815	4	423766	15	NULL	NULL	0	NULL	asthmatic airway smooth muscle-conditioned medium	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As predicted from the role of KCa3 .1 in HLMC migration , adenosine abolished HLMC chemotaxis to asthmatic airway smooth muscle-conditioned medium .
	manualset3
242816	1	423767	15	NULL	NULL	0	NULL	fluorescence	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	As shown in fluorescence , the red emissions attributed to ( 5 ) D ( 0 ) - ( 7 ) F ( J ) transitions ( J = 1 , 2 , 3 , 4 ) of Eu ( 3 + ) ions were quenched by the phenylalanine ( Phe ) , and a strong blue emission at around 445 nm appeared .
	manualset3
242817	2	423767	15	NULL	NULL	0	NULL	red emissions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As shown in fluorescence , the red emissions attributed to ( 5 ) D ( 0 ) - ( 7 ) F ( J ) transitions ( J = 1 , 2 , 3 , 4 ) of Eu ( 3 + ) ions were quenched by the phenylalanine ( Phe ) , and a strong blue emission at around 445 nm appeared .
	manualset3
242818	3	423767	15	NULL	NULL	NULL	NULL	( 5 ) D ( 0 ) - ( 7 ) F ( J ) transitions ( J = 1 , 2 , 3 , 4 ) 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As shown in fluorescence , the red emissions attributed to ( 5 ) D ( 0 ) - ( 7 ) F ( J ) transitions ( J = 1 , 2 , 3 , 4 ) of Eu ( 3 + ) ions were quenched by the phenylalanine ( Phe ) , and a strong blue emission at around 445 nm appeared .
	manualset3
242819	4	423767	15	NULL	NULL	0	NULL	Eu ( 3 + ) ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	As shown in fluorescence , the red emissions attributed to ( 5 ) D ( 0 ) - ( 7 ) F ( J ) transitions ( J = 1 , 2 , 3 , 4 ) of Eu ( 3 + ) ions were quenched by the phenylalanine ( Phe ) , and a strong blue emission at around 445 nm appeared .
	manualset3
242820	5	423767	15	NULL	NULL	0	NULL	phenylalanine ( Phe )	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	As shown in fluorescence , the red emissions attributed to ( 5 ) D ( 0 ) - ( 7 ) F ( J ) transitions ( J = 1 , 2 , 3 , 4 ) of Eu ( 3 + ) ions were quenched by the phenylalanine ( Phe ) , and a strong blue emission at around 445 nm appeared .
	manualset3
242821	6	423767	15	NULL	NULL	0	NULL	blue emission	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As shown in fluorescence , the red emissions attributed to ( 5 ) D ( 0 ) - ( 7 ) F ( J ) transitions ( J = 1 , 2 , 3 , 4 ) of Eu ( 3 + ) ions were quenched by the phenylalanine ( Phe ) , and a strong blue emission at around 445 nm appeared .
	manualset3
242822	7	423767	15	NULL	NULL	0	NULL	445 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As shown in fluorescence , the red emissions attributed to ( 5 ) D ( 0 ) - ( 7 ) F ( J ) transitions ( J = 1 , 2 , 3 , 4 ) of Eu ( 3 + ) ions were quenched by the phenylalanine ( Phe ) , and a strong blue emission at around 445 nm appeared .
	manualset3
242823	1	423768	15	NULL	NULL	0	NULL	Effects of food legislation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of food legislation on the hygienic production of milk and milk products ) .
	manualset3
242824	2	423768	15	NULL	NULL	0	NULL	hygienic production of milk	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of food legislation on the hygienic production of milk and milk products ) .
	manualset3
242825	3	423768	15	NULL	NULL	0	NULL	 milk products	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of food legislation on the hygienic production of milk and milk products ) .
	manualset3
242826	1	423769	15	NULL	NULL	NULL	NULL	behavioral medicine	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As with behavioral medicine , alternative medicine does not fit into the systems developed for delivering medical-surgical services .
	manualset3
242827	2	423769	15	NULL	NULL	0	NULL	alternative medicine	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	As with behavioral medicine , alternative medicine does not fit into the systems developed for delivering medical-surgical services .
	manualset3
242828	3	423769	15	NULL	NULL	0	NULL	systems	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As with behavioral medicine , alternative medicine does not fit into the systems developed for delivering medical-surgical services .
	manualset3
242829	4	423769	15	NULL	NULL	0	NULL	delivering medical-surgical services 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	As with behavioral medicine , alternative medicine does not fit into the systems developed for delivering medical-surgical services .
	manualset3
242830	1	423770	15	NULL	NULL	0	NULL	cisplatin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	As expected , cisplatin also increased the number of c-fos-positive cells in these regions .
	manualset3
242831	2	423770	15	NULL	NULL	0	NULL	number 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As expected , cisplatin also increased the number of c-fos-positive cells in these regions .
	manualset3
242832	3	423770	15	NULL	NULL	0	NULL	c-fos-positive cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	As expected , cisplatin also increased the number of c-fos-positive cells in these regions .
	manualset3
242833	4	423770	15	NULL	NULL	NULL	NULL	regions	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As expected , cisplatin also increased the number of c-fos-positive cells in these regions .
	manualset3
242834	1	423771	15	NULL	NULL	0	NULL	copper deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As expected , copper deficiency dramatically reduced SOD .
	manualset3
242835	2	423771	15	NULL	NULL	0	NULL	SOD	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	As expected , copper deficiency dramatically reduced SOD .
	manualset3
242836	1	423772	15	NULL	NULL	0	NULL	strains that over-produce OmpT 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	As expected , strains that over-produce OmpT are less susceptible to infection by ColE2 than by ColE2-Im2 .
	manualset3
242837	2	423772	15	NULL	NULL	0	NULL	infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As expected , strains that over-produce OmpT are less susceptible to infection by ColE2 than by ColE2-Im2 .
	manualset3
242838	3	423772	15	NULL	NULL	0	NULL	ColE2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	As expected , strains that over-produce OmpT are less susceptible to infection by ColE2 than by ColE2-Im2 .
	manualset3
242839	4	423772	15	NULL	NULL	0	NULL	ColE2-Im2	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As expected , strains that over-produce OmpT are less susceptible to infection by ColE2 than by ColE2-Im2 .
	manualset3
242841	1	423773	15	NULL	NULL	0	NULL	static lung volumes	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As expected , we found higher static and dynamic ( FVC , FEV1 , PEF ) lung volumes in boys than in girls relating to height .
	manualset3
242842	2	423773	15	NULL	NULL	0	NULL	dynamic lung volumes 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As expected , we found higher static and dynamic ( FVC , FEV1 , PEF ) lung volumes in boys than in girls relating to height .
	manualset3
242843	3	423773	15	NULL	NULL	0	NULL	FVC	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As expected , we found higher static and dynamic ( FVC , FEV1 , PEF ) lung volumes in boys than in girls relating to height .
	manualset3
242844	4	423773	15	NULL	NULL	0	NULL	FEV1	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As expected , we found higher static and dynamic ( FVC , FEV1 , PEF ) lung volumes in boys than in girls relating to height .
	manualset3
242845	5	423773	15	NULL	NULL	0	NULL	PEF	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As expected , we found higher static and dynamic ( FVC , FEV1 , PEF ) lung volumes in boys than in girls relating to height .
	manualset3
242846	6	423773	15	NULL	NULL	0	NULL	boys	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As expected , we found higher static and dynamic ( FVC , FEV1 , PEF ) lung volumes in boys than in girls relating to height .
	manualset3
242847	7	423773	15	NULL	NULL	0	NULL	girls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As expected , we found higher static and dynamic ( FVC , FEV1 , PEF ) lung volumes in boys than in girls relating to height .
	manualset3
242848	8	423773	15	NULL	NULL	0	NULL	height	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As expected , we found higher static and dynamic ( FVC , FEV1 , PEF ) lung volumes in boys than in girls relating to height .
	manualset3
242849	1	423774	15	NULL	NULL	0	NULL	biologic data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	As far as biologic data are concerned , some elements point to the role of H. pylori in the development of preneoplastic and neoplastic changes , such as intestinal metaplasia and dysplasia .
	manualset3
242850	2	423774	15	NULL	NULL	0	NULL	elements	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	As far as biologic data are concerned , some elements point to the role of H. pylori in the development of preneoplastic and neoplastic changes , such as intestinal metaplasia and dysplasia .
	manualset3
242851	3	423774	15	NULL	NULL	0	NULL	role of H. pylori 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As far as biologic data are concerned , some elements point to the role of H. pylori in the development of preneoplastic and neoplastic changes , such as intestinal metaplasia and dysplasia .
	manualset3
242852	4	423774	15	NULL	NULL	NULL	NULL	development of preneoplastic changes	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As far as biologic data are concerned , some elements point to the role of H. pylori in the development of preneoplastic and neoplastic changes , such as intestinal metaplasia and dysplasia .
	manualset3
242854	5	423774	15	NULL	NULL	0	NULL	development of neoplastic changes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As far as biologic data are concerned , some elements point to the role of H. pylori in the development of preneoplastic and neoplastic changes , such as intestinal metaplasia and dysplasia .
	manualset3
242855	6	423774	15	NULL	NULL	0	NULL	intestinal metaplasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As far as biologic data are concerned , some elements point to the role of H. pylori in the development of preneoplastic and neoplastic changes , such as intestinal metaplasia and dysplasia .
	manualset3
242856	7	423774	15	NULL	NULL	0	NULL	dysplasia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As far as biologic data are concerned , some elements point to the role of H. pylori in the development of preneoplastic and neoplastic changes , such as intestinal metaplasia and dysplasia .
	manualset3
242857	1	423775	15	NULL	NULL	0	NULL	 specificity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As to specificity , other PP2A regulatory subunits had negligible effects on TH activity and phosphorylation in situ and in vitro .
	manualset3
242858	2	423775	15	NULL	NULL	0	NULL	PP2A regulatory subunits	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As to specificity , other PP2A regulatory subunits had negligible effects on TH activity and phosphorylation in situ and in vitro .
	manualset3
242859	3	423775	15	NULL	NULL	0	NULL	effects on TH activity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As to specificity , other PP2A regulatory subunits had negligible effects on TH activity and phosphorylation in situ and in vitro .
	manualset3
242860	4	423775	15	NULL	NULL	0	NULL	phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As to specificity , other PP2A regulatory subunits had negligible effects on TH activity and phosphorylation in situ and in vitro .
	manualset3
242861	1	423776	15	NULL	NULL	0	NULL	substrate	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	As well as being a substrate for the enzymes phospholipase C ( PLC ) and phosphatidylinositol 3-kinase ( PI3K ) , PtdIns ( 4 , 5 ) P ( 2 ) acts as a second messenger in its own right , influencing a variety of cellular processes .
	manualset3
242862	2	423776	15	NULL	NULL	0	NULL	enzymes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As well as being a substrate for the enzymes phospholipase C ( PLC ) and phosphatidylinositol 3-kinase ( PI3K ) , PtdIns ( 4 , 5 ) P ( 2 ) acts as a second messenger in its own right , influencing a variety of cellular processes .
	manualset3
242863	3	423776	15	NULL	NULL	0	NULL	phospholipase C ( PLC )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	As well as being a substrate for the enzymes phospholipase C ( PLC ) and phosphatidylinositol 3-kinase ( PI3K ) , PtdIns ( 4 , 5 ) P ( 2 ) acts as a second messenger in its own right , influencing a variety of cellular processes .
	manualset3
242864	4	423776	15	NULL	NULL	0	NULL	phosphatidylinositol 3-kinase ( PI3K ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	As well as being a substrate for the enzymes phospholipase C ( PLC ) and phosphatidylinositol 3-kinase ( PI3K ) , PtdIns ( 4 , 5 ) P ( 2 ) acts as a second messenger in its own right , influencing a variety of cellular processes .
	manualset3
242865	5	423776	15	NULL	NULL	0	NULL	PtdIns ( 4 , 5 ) P ( 2 ) 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	As well as being a substrate for the enzymes phospholipase C ( PLC ) and phosphatidylinositol 3-kinase ( PI3K ) , PtdIns ( 4 , 5 ) P ( 2 ) acts as a second messenger in its own right , influencing a variety of cellular processes .
	manualset3
242866	6	423776	15	NULL	NULL	NULL	NULL	second messenger	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As well as being a substrate for the enzymes phospholipase C ( PLC ) and phosphatidylinositol 3-kinase ( PI3K ) , PtdIns ( 4 , 5 ) P ( 2 ) acts as a second messenger in its own right , influencing a variety of cellular processes .
	manualset3
242867	7	423776	15	NULL	NULL	0	NULL	right	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As well as being a substrate for the enzymes phospholipase C ( PLC ) and phosphatidylinositol 3-kinase ( PI3K ) , PtdIns ( 4 , 5 ) P ( 2 ) acts as a second messenger in its own right , influencing a variety of cellular processes .
	manualset3
242868	8	423776	15	NULL	NULL	0	NULL	cellular processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As well as being a substrate for the enzymes phospholipase C ( PLC ) and phosphatidylinositol 3-kinase ( PI3K ) , PtdIns ( 4 , 5 ) P ( 2 ) acts as a second messenger in its own right , influencing a variety of cellular processes .
	manualset3
242869	1	423777	15	NULL	NULL	0	NULL	Effects of photocoagulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of photocoagulation on the velocity of retinal circulation in diabetic retinopathy ( author 's transl ) ) .
	manualset3
242870	2	423777	15	NULL	NULL	0	NULL	velocity of retinal circulation 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of photocoagulation on the velocity of retinal circulation in diabetic retinopathy ( author 's transl ) ) .
	manualset3
242871	3	423777	15	NULL	NULL	NULL	NULL	diabetic retinopathy 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Effects of photocoagulation on the velocity of retinal circulation in diabetic retinopathy ( author 's transl ) ) .
	manualset3
242938	4	423777	15	NULL	NULL	NULL	NULL	author 's transl 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Effects of photocoagulation on the velocity of retinal circulation in diabetic retinopathy ( author 's transl ) ) .
	manualset3
242872	1	423778	15	NULL	NULL	NULL	NULL	experiments	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As well as in our experiments , severe stenosis had been reported in several animal studies .
	manualset3
242873	2	423778	15	NULL	NULL	0	NULL	stenosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As well as in our experiments , severe stenosis had been reported in several animal studies .
	manualset3
242874	3	423778	15	NULL	NULL	0	NULL	animal studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	As well as in our experiments , severe stenosis had been reported in several animal studies .
	manualset3
242875	1	423779	15	NULL	NULL	0	NULL	lung cancer patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As it was previously established for lung cancer patients treated with living BCG , in the group of sparing scheme-treated patients the longest survival period pertained to patients treated once and patients treated twice or three times and an inverse correlation existed between the number of applications of F70 and the mean survival period .
	manualset3
242876	2	423779	15	NULL	NULL	0	NULL	living BCG	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	As it was previously established for lung cancer patients treated with living BCG , in the group of sparing scheme-treated patients the longest survival period pertained to patients treated once and patients treated twice or three times and an inverse correlation existed between the number of applications of F70 and the mean survival period .
	manualset3
242877	3	423779	15	NULL	NULL	0	NULL	group of sparing scheme-treated patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As it was previously established for lung cancer patients treated with living BCG , in the group of sparing scheme-treated patients the longest survival period pertained to patients treated once and patients treated twice or three times and an inverse correlation existed between the number of applications of F70 and the mean survival period .
	manualset3
242878	4	423779	15	NULL	NULL	NULL	NULL	survival period	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As it was previously established for lung cancer patients treated with living BCG , in the group of sparing scheme-treated patients the longest survival period pertained to patients treated once and patients treated twice or three times and an inverse correlation existed between the number of applications of F70 and the mean survival period .
	manualset3
242879	5	423779	15	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As it was previously established for lung cancer patients treated with living BCG , in the group of sparing scheme-treated patients the longest survival period pertained to patients treated once and patients treated twice or three times and an inverse correlation existed between the number of applications of F70 and the mean survival period .
	manualset3
242881	6	423779	15	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As it was previously established for lung cancer patients treated with living BCG , in the group of sparing scheme-treated patients the longest survival period pertained to patients treated once and patients treated twice or three times and an inverse correlation existed between the number of applications of F70 and the mean survival period .
	manualset3
242882	7	423779	15	NULL	NULL	0	NULL	inverse correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	As it was previously established for lung cancer patients treated with living BCG , in the group of sparing scheme-treated patients the longest survival period pertained to patients treated once and patients treated twice or three times and an inverse correlation existed between the number of applications of F70 and the mean survival period .
	manualset3
242883	8	423779	15	NULL	NULL	0	NULL	number of applications of F70	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	As it was previously established for lung cancer patients treated with living BCG , in the group of sparing scheme-treated patients the longest survival period pertained to patients treated once and patients treated twice or three times and an inverse correlation existed between the number of applications of F70 and the mean survival period .
	manualset3
242884	9	423779	15	NULL	NULL	0	NULL	mean survival period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	As it was previously established for lung cancer patients treated with living BCG , in the group of sparing scheme-treated patients the longest survival period pertained to patients treated once and patients treated twice or three times and an inverse correlation existed between the number of applications of F70 and the mean survival period .
	manualset3
242885	1	423780	15	NULL	NULL	0	NULL	reference	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As reference , antibodies against the holoenzyme and the CA2 + - transport ATPase of sarcoplasmic reticulum were induced .
	manualset3
242886	2	423780	15	NULL	NULL	0	NULL	antibodies against the holoenzyme 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As reference , antibodies against the holoenzyme and the CA2 + - transport ATPase of sarcoplasmic reticulum were induced .
	manualset3
242887	3	423780	15	NULL	NULL	0	NULL	CA2 + - transport ATPase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	As reference , antibodies against the holoenzyme and the CA2 + - transport ATPase of sarcoplasmic reticulum were induced .
	manualset3
242888	4	423780	15	NULL	NULL	0	NULL	sarcoplasmic reticulum	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	As reference , antibodies against the holoenzyme and the CA2 + - transport ATPase of sarcoplasmic reticulum were induced .
	manualset3
242889	1	423781	15	NULL	NULL	NULL	NULL	understanding	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As such , an understanding of the mechanisms governing adipose tissue differentiation and function is of considerable importance .
	manualset3
242890	2	423781	15	NULL	NULL	0	NULL	mechanisms governing adipose tissue differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As such , an understanding of the mechanisms governing adipose tissue differentiation and function is of considerable importance .
	manualset3
242891	3	423781	15	NULL	NULL	0	NULL	function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As such , an understanding of the mechanisms governing adipose tissue differentiation and function is of considerable importance .
	manualset3
242892	4	423781	15	NULL	NULL	0	NULL	importance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	As such , an understanding of the mechanisms governing adipose tissue differentiation and function is of considerable importance .
	manualset3
242893	1	423782	15	NULL	NULL	0	NULL	therapeutic agent	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	As such , it could be a useful therapeutic agent to antagonize the tumor-promoting activity of TGF-beta .
	manualset3
242894	2	423782	15	NULL	NULL	0	NULL	antagonize the tumor-promoting activity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As such , it could be a useful therapeutic agent to antagonize the tumor-promoting activity of TGF-beta .
	manualset3
242895	3	423782	15	NULL	NULL	0	NULL	TGF-beta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	As such , it could be a useful therapeutic agent to antagonize the tumor-promoting activity of TGF-beta .
	manualset3
242896	1	423783	15	NULL	NULL	0	NULL	substrate	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	As the preferred substrate this activity acetylates oligopeptides with N termini Met-Leu-Xxx-Pro .
	manualset3
242897	2	423783	15	NULL	NULL	0	NULL	activity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As the preferred substrate this activity acetylates oligopeptides with N termini Met-Leu-Xxx-Pro .
	manualset3
242898	3	423783	15	NULL	NULL	0	NULL	oligopeptides	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	As the preferred substrate this activity acetylates oligopeptides with N termini Met-Leu-Xxx-Pro .
	manualset3
242900	4	423783	15	NULL	NULL	0	NULL	N termini Met-Leu-Xxx-Pro	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	As the preferred substrate this activity acetylates oligopeptides with N termini Met-Leu-Xxx-Pro .
	manualset3
242901	1	423784	15	NULL	NULL	0	NULL	risk of developing antibiotic resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As there is a risk of developing antibiotic resistance , a number of commonly-used antimicrobial growth promoters have been banned in the EU member states .
	manualset3
242902	2	423784	15	NULL	NULL	0	NULL	number of commonly-used antimicrobial growth promoters	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	As there is a risk of developing antibiotic resistance , a number of commonly-used antimicrobial growth promoters have been banned in the EU member states .
	manualset3
242903	3	423784	15	NULL	NULL	0	NULL	EU member states	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	As there is a risk of developing antibiotic resistance , a number of commonly-used antimicrobial growth promoters have been banned in the EU member states .
	manualset3
242904	1	423785	15	NULL	NULL	NULL	NULL	glial contributions to synapse formation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	As we continue to learn about glial contributions to synapse formation and maintenance , it is likely that glia-derived signals will emerge as potential therapeutic targets for diseases that involve aberrant circuit function such as autism , epilepsy and Alzheimer 's Disease .
	manualset3
242905	2	423785	15	NULL	NULL	0	NULL	synapse maintenance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As we continue to learn about glial contributions to synapse formation and maintenance , it is likely that glia-derived signals will emerge as potential therapeutic targets for diseases that involve aberrant circuit function such as autism , epilepsy and Alzheimer 's Disease .
	manualset3
242906	3	423785	15	NULL	NULL	0	NULL	glia-derived signals 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As we continue to learn about glial contributions to synapse formation and maintenance , it is likely that glia-derived signals will emerge as potential therapeutic targets for diseases that involve aberrant circuit function such as autism , epilepsy and Alzheimer 's Disease .
	manualset3
242907	4	423785	15	NULL	NULL	0	NULL	potential therapeutic targets	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	As we continue to learn about glial contributions to synapse formation and maintenance , it is likely that glia-derived signals will emerge as potential therapeutic targets for diseases that involve aberrant circuit function such as autism , epilepsy and Alzheimer 's Disease .
	manualset3
242908	5	423785	15	NULL	NULL	0	NULL	diseases 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	As we continue to learn about glial contributions to synapse formation and maintenance , it is likely that glia-derived signals will emerge as potential therapeutic targets for diseases that involve aberrant circuit function such as autism , epilepsy and Alzheimer 's Disease .
	manualset3
242909	6	423785	15	NULL	NULL	0	NULL	aberrant circuit function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	As we continue to learn about glial contributions to synapse formation and maintenance , it is likely that glia-derived signals will emerge as potential therapeutic targets for diseases that involve aberrant circuit function such as autism , epilepsy and Alzheimer 's Disease .
	manualset3
242910	7	423785	15	NULL	NULL	0	NULL	autism	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	As we continue to learn about glial contributions to synapse formation and maintenance , it is likely that glia-derived signals will emerge as potential therapeutic targets for diseases that involve aberrant circuit function such as autism , epilepsy and Alzheimer 's Disease .
	manualset3
242911	8	423785	15	NULL	NULL	0	NULL	epilepsy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	As we continue to learn about glial contributions to synapse formation and maintenance , it is likely that glia-derived signals will emerge as potential therapeutic targets for diseases that involve aberrant circuit function such as autism , epilepsy and Alzheimer 's Disease .
	manualset3
242912	9	423785	15	NULL	NULL	0	NULL	Alzheimer 's Disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	As we continue to learn about glial contributions to synapse formation and maintenance , it is likely that glia-derived signals will emerge as potential therapeutic targets for diseases that involve aberrant circuit function such as autism , epilepsy and Alzheimer 's Disease .
	manualset3
242913	1	423786	15	NULL	NULL	0	NULL	Ascending back pain 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ascending back pain and headache during attempted epidural placement .
	manualset3
242914	2	423786	15	NULL	NULL	0	NULL	headache	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Ascending back pain and headache during attempted epidural placement .
	manualset3
242915	3	423786	15	NULL	NULL	0	NULL	epidural placement	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Ascending back pain and headache during attempted epidural placement .
	manualset3
242916	1	423787	15	NULL	NULL	0	NULL	Ascorbic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ascorbic acid enhanced the absorption of both metal ions , while NaF ( 1 mM ) as an inhibitor of glycolytic energy supply , decreased their absorption .
	manualset3
242917	2	423787	15	NULL	NULL	0	NULL	absorption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ascorbic acid enhanced the absorption of both metal ions , while NaF ( 1 mM ) as an inhibitor of glycolytic energy supply , decreased their absorption .
	manualset3
242918	3	423787	15	NULL	NULL	0	NULL	metal ions	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Ascorbic acid enhanced the absorption of both metal ions , while NaF ( 1 mM ) as an inhibitor of glycolytic energy supply , decreased their absorption .
	manualset3
242919	4	423787	15	NULL	NULL	0	NULL	NaF ( 1 mM )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Ascorbic acid enhanced the absorption of both metal ions , while NaF ( 1 mM ) as an inhibitor of glycolytic energy supply , decreased their absorption .
	manualset3
242920	5	423787	15	NULL	NULL	0	NULL	inhibitor of glycolytic energy supply	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ascorbic acid enhanced the absorption of both metal ions , while NaF ( 1 mM ) as an inhibitor of glycolytic energy supply , decreased their absorption .
	manualset3
242921	6	423787	15	NULL	NULL	0	NULL	absorption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ascorbic acid enhanced the absorption of both metal ions , while NaF ( 1 mM ) as an inhibitor of glycolytic energy supply , decreased their absorption .
	manualset3
242922	1	423788	15	NULL	NULL	0	NULL	Ascorbic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ascorbic acid stimulated ECM secretion ( collagen and glycosaminoglycan ) and cell proliferation .
	manualset3
242923	2	423788	15	NULL	NULL	0	NULL	ECM secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ascorbic acid stimulated ECM secretion ( collagen and glycosaminoglycan ) and cell proliferation .
	manualset3
242924	3	423788	15	NULL	NULL	0	NULL	collagen	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ascorbic acid stimulated ECM secretion ( collagen and glycosaminoglycan ) and cell proliferation .
	manualset3
242925	4	423788	15	NULL	NULL	0	NULL	glycosaminoglycan	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Ascorbic acid stimulated ECM secretion ( collagen and glycosaminoglycan ) and cell proliferation .
	manualset3
242926	5	423788	15	NULL	NULL	0	NULL	cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ascorbic acid stimulated ECM secretion ( collagen and glycosaminoglycan ) and cell proliferation .
	manualset3
242927	1	423789	15	NULL	NULL	0	NULL	Aspartate levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Aspartate levels were also significantly reduced ( by 32 to 35 % ) in the spinal cord only .
	manualset3
242928	2	423789	15	NULL	NULL	0	NULL	32 to 35 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Aspartate levels were also significantly reduced ( by 32 to 35 % ) in the spinal cord only .
	manualset3
242929	3	423789	15	NULL	NULL	0	NULL	spinal cord	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Aspartate levels were also significantly reduced ( by 32 to 35 % ) in the spinal cord only .
	manualset3
242930	1	423790	15	NULL	NULL	0	NULL	Aspartate	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Aspartate was a non-competitive inhibitor of PEP-C activity .
	manualset3
242931	2	423790	15	NULL	NULL	0	NULL	non-competitive inhibitor of PEP-C activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Aspartate was a non-competitive inhibitor of PEP-C activity .
	manualset3
242932	1	423791	15	NULL	NULL	0	NULL	Effects of transmural electrical stimulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of transmural electrical stimulation , raising of intraluminal pressure and application of some drugs on motility and intracellular potentials of the chicken bile duct ( author 's transl ) ) .
	manualset3
242933	2	423791	15	NULL	NULL	0	NULL	intraluminal pressure 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of transmural electrical stimulation , raising of intraluminal pressure and application of some drugs on motility and intracellular potentials of the chicken bile duct ( author 's transl ) ) .
	manualset3
242934	3	423791	15	NULL	NULL	0	NULL	application of some drugs	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of transmural electrical stimulation , raising of intraluminal pressure and application of some drugs on motility and intracellular potentials of the chicken bile duct ( author 's transl ) ) .
	manualset3
242935	4	423791	15	NULL	NULL	0	NULL	motility	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of transmural electrical stimulation , raising of intraluminal pressure and application of some drugs on motility and intracellular potentials of the chicken bile duct ( author 's transl ) ) .
	manualset3
242936	5	423791	15	NULL	NULL	0	NULL	intracellular potentials 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of transmural electrical stimulation , raising of intraluminal pressure and application of some drugs on motility and intracellular potentials of the chicken bile duct ( author 's transl ) ) .
	manualset3
242939	6	423791	15	NULL	NULL	0	NULL	chicken bile duct 													NULL		0	NULL	NULL	NULL	NULL	NULL	( Effects of transmural electrical stimulation , raising of intraluminal pressure and application of some drugs on motility and intracellular potentials of the chicken bile duct ( author 's transl ) ) .
	manualset3
242940	7	423791	15	NULL	NULL	NULL	NULL	author 's transl	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Effects of transmural electrical stimulation , raising of intraluminal pressure and application of some drugs on motility and intracellular potentials of the chicken bile duct ( author 's transl ) ) .
	manualset3
242941	1	423792	15	NULL	NULL	0	NULL	Aspects of rural social milieu 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Aspects of rural social milieu may help to keep mental HRQOL high , even in the face of severe chronic disease .
	manualset3
242942	2	423792	15	NULL	NULL	0	NULL	mental HRQOL	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Aspects of rural social milieu may help to keep mental HRQOL high , even in the face of severe chronic disease .
	manualset3
242943	3	423792	15	NULL	NULL	0	NULL	face of severe chronic disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Aspects of rural social milieu may help to keep mental HRQOL high , even in the face of severe chronic disease .
	manualset3
242944	1	423793	15	NULL	NULL	NULL	NULL	Aspects of the pathology 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Aspects of the pathology of stifle bone cysts in the horse .
	manualset3
242945	2	423793	15	NULL	NULL	0	NULL	stifle bone cysts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Aspects of the pathology of stifle bone cysts in the horse .
	manualset3
242946	3	423793	15	NULL	NULL	0	NULL	 horse	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Aspects of the pathology of stifle bone cysts in the horse .
	manualset3
242947	1	423794	15	NULL	NULL	0	NULL	Aspirin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Aspirin did not inhibit white body formation but another non-steroid anti-inflammatory agent , flurbiprofen was able to do so , as was the anti-gout agent , sulphinpyrazone .
	manualset3
242948	2	423794	15	NULL	NULL	0	NULL	white body formation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Aspirin did not inhibit white body formation but another non-steroid anti-inflammatory agent , flurbiprofen was able to do so , as was the anti-gout agent , sulphinpyrazone .
	manualset3
242949	3	423794	15	NULL	NULL	0	NULL	non-steroid anti-inflammatory agent	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Aspirin did not inhibit white body formation but another non-steroid anti-inflammatory agent , flurbiprofen was able to do so , as was the anti-gout agent , sulphinpyrazone .
	manualset3
242950	4	423794	15	NULL	NULL	0	NULL	flurbiprofen 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Aspirin did not inhibit white body formation but another non-steroid anti-inflammatory agent , flurbiprofen was able to do so , as was the anti-gout agent , sulphinpyrazone .
	manualset3
242951	5	423794	15	NULL	NULL	0	NULL	anti-gout agent	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Aspirin did not inhibit white body formation but another non-steroid anti-inflammatory agent , flurbiprofen was able to do so , as was the anti-gout agent , sulphinpyrazone .
	manualset3
242952	6	423794	15	NULL	NULL	0	NULL	sulphinpyrazone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Aspirin did not inhibit white body formation but another non-steroid anti-inflammatory agent , flurbiprofen was able to do so , as was the anti-gout agent , sulphinpyrazone .
	manualset3
242953	1	423795	15	NULL	NULL	0	NULL	Aspirin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Aspirin promotes TFF2 gene activation in human gastric cancer cell lines .
	manualset3
242954	2	423795	15	NULL	NULL	0	NULL	TFF2 gene activation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Aspirin promotes TFF2 gene activation in human gastric cancer cell lines .
	manualset3
242955	3	423795	15	NULL	NULL	0	NULL	human gastric cancer cell lines 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Aspirin promotes TFF2 gene activation in human gastric cancer cell lines .
	manualset3
242956	1	423796	15	NULL	NULL	0	NULL	Assay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Assay and purity control of minocycline by thin-layer chromatography using UV and fluorescence densitometry -- a comparison with liquid chromatography .
	manualset3
242957	2	423796	15	NULL	NULL	0	NULL	purity control of minocycline by thin-layer chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Assay and purity control of minocycline by thin-layer chromatography using UV and fluorescence densitometry -- a comparison with liquid chromatography .
	manualset3
242958	3	423796	15	NULL	NULL	0	NULL	UV densitometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Assay and purity control of minocycline by thin-layer chromatography using UV and fluorescence densitometry -- a comparison with liquid chromatography .
	manualset3
242959	4	423796	15	NULL	NULL	0	NULL	fluorescence densitometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Assay and purity control of minocycline by thin-layer chromatography using UV and fluorescence densitometry -- a comparison with liquid chromatography .
	manualset3
242960	5	423796	15	NULL	NULL	0	NULL	comparison 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Assay and purity control of minocycline by thin-layer chromatography using UV and fluorescence densitometry -- a comparison with liquid chromatography .
	manualset3
242961	6	423796	15	NULL	NULL	0	NULL	liquid chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Assay and purity control of minocycline by thin-layer chromatography using UV and fluorescence densitometry -- a comparison with liquid chromatography .
	manualset3
242962	1	423797	15	NULL	NULL	0	NULL	Assays 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Assays of sex-related hormones showed a significant decrease in only the estradiol serum level at days 3 and 7 , as compared with the control group .
	manualset3
242963	2	423797	15	NULL	NULL	0	NULL	sex-related hormones	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Assays of sex-related hormones showed a significant decrease in only the estradiol serum level at days 3 and 7 , as compared with the control group .
	manualset3
242964	3	423797	15	NULL	NULL	0	NULL	decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Assays of sex-related hormones showed a significant decrease in only the estradiol serum level at days 3 and 7 , as compared with the control group .
	manualset3
242965	4	423797	15	NULL	NULL	0	NULL	estradiol serum level 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Assays of sex-related hormones showed a significant decrease in only the estradiol serum level at days 3 and 7 , as compared with the control group .
	manualset3
242966	5	423797	15	NULL	NULL	0	NULL	days 3	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Assays of sex-related hormones showed a significant decrease in only the estradiol serum level at days 3 and 7 , as compared with the control group .
	manualset3
242967	6	423797	15	NULL	NULL	0	NULL	days 7	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Assays of sex-related hormones showed a significant decrease in only the estradiol serum level at days 3 and 7 , as compared with the control group .
	manualset3
242968	7	423797	15	NULL	NULL	0	NULL	control group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Assays of sex-related hormones showed a significant decrease in only the estradiol serum level at days 3 and 7 , as compared with the control group .
	manualset3
242969	1	423798	15	NULL	NULL	0	NULL	Assembly	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Assembly of vesicular stomatitis virus nucleocapsids in vivo : a kinetic analysis .
	manualset3
242970	2	423798	15	NULL	NULL	0	NULL	vesicular stomatitis virus nucleocapsids 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Assembly of vesicular stomatitis virus nucleocapsids in vivo : a kinetic analysis .
	manualset3
242971	3	423798	15	NULL	NULL	0	NULL	kinetic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Assembly of vesicular stomatitis virus nucleocapsids in vivo : a kinetic analysis .
	manualset3
242972	1	423799	15	NULL	NULL	0	NULL	Assembly of the mature TCR complex 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Assembly of the mature TCR complex requires specific subunit interactions , the detailed nature of which is becoming more evident .
	manualset3
242973	2	423799	15	NULL	NULL	0	NULL	specific subunit interactions	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Assembly of the mature TCR complex requires specific subunit interactions , the detailed nature of which is becoming more evident .
	manualset3
242974	3	423799	15	NULL	NULL	0	NULL	nature	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Assembly of the mature TCR complex requires specific subunit interactions , the detailed nature of which is becoming more evident .
	manualset3
242975	1	423800	15	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Assess patients with major depression or substance abuse for suicide ideation , as they are at elevated risk for self-harm .
	manualset3
242976	2	423800	15	NULL	NULL	0	NULL	depression	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Assess patients with major depression or substance abuse for suicide ideation , as they are at elevated risk for self-harm .
	manualset3
242977	3	423800	15	NULL	NULL	0	NULL	substance abuse	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Assess patients with major depression or substance abuse for suicide ideation , as they are at elevated risk for self-harm .
	manualset3
242978	4	423800	15	NULL	NULL	0	NULL	suicide ideation	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Assess patients with major depression or substance abuse for suicide ideation , as they are at elevated risk for self-harm .
	manualset3
242979	5	423800	15	NULL	NULL	0	NULL	risk for self-harm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Assess patients with major depression or substance abuse for suicide ideation , as they are at elevated risk for self-harm .
	manualset3
242980	1	423801	15	NULL	NULL	0	NULL	Assessing quality of microarrays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessing quality and normalization of microarrays : case studies using neurological genomic data .
	manualset3
242981	2	423801	15	NULL	NULL	0	NULL	normalization of microarrays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessing quality and normalization of microarrays : case studies using neurological genomic data .
	manualset3
242982	3	423801	15	NULL	NULL	0	NULL	case studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessing quality and normalization of microarrays : case studies using neurological genomic data .
	manualset3
242983	4	423801	15	NULL	NULL	0	NULL	neurological genomic data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessing quality and normalization of microarrays : case studies using neurological genomic data .
	manualset3
242984	1	423802	15	NULL	NULL	0	NULL	Assessing the functional status	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessing the functional status of the older adult requires evaluation of both the person and the environment .
	manualset3
242985	2	423802	15	NULL	NULL	0	NULL	older adult	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessing the functional status of the older adult requires evaluation of both the person and the environment .
	manualset3
242986	3	423802	15	NULL	NULL	0	NULL	evaluation of person	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessing the functional status of the older adult requires evaluation of both the person and the environment .
	manualset3
242987	4	423802	15	NULL	NULL	0	NULL	evaluation of the environment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessing the functional status of the older adult requires evaluation of both the person and the environment .
	manualset3
242988	1	423803	15	NULL	NULL	0	NULL	Assessing the results	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessing the results of laser treatment of port-wine stains ( PWS ) is very subjective .
	manualset3
242989	2	423803	15	NULL	NULL	NULL	NULL	laser treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Assessing the results of laser treatment of port-wine stains ( PWS ) is very subjective .
	manualset3
242990	3	423803	15	NULL	NULL	0	NULL	port-wine stains ( PWS )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessing the results of laser treatment of port-wine stains ( PWS ) is very subjective .
	manualset3
243014	1	423804	15	NULL	NULL	0	NULL	Assessment of a two-generation reproductive study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of a two-generation reproductive and fertility study of mercuric chloride in rats .
	manualset3
243074	2	423804	15	NULL	NULL	0	NULL	fertility study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of a two-generation reproductive and fertility study of mercuric chloride in rats .
	manualset3
243075	3	423804	15	NULL	NULL	0	NULL	mercuric chloride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of a two-generation reproductive and fertility study of mercuric chloride in rats .
	manualset3
243076	4	423804	15	NULL	NULL	0	NULL	rats 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of a two-generation reproductive and fertility study of mercuric chloride in rats .
	manualset3
243077	1	423805	15	NULL	NULL	0	NULL	Assessment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of an on-line computerized perinatal data collection and information system .
	manualset3
243078	2	423805	15	NULL	NULL	NULL	NULL	on-line computerized perinatal data collection	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Assessment of an on-line computerized perinatal data collection and information system .
	manualset3
243082	3	423805	15	NULL	NULL	0	NULL	information system	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of an on-line computerized perinatal data collection and information system .
	manualset3
243083	1	423806	15	NULL	NULL	0	NULL	Assessment of anatomy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of anatomy and cardiac function by Doppler echocardiography .
	manualset3
243084	2	423806	15	NULL	NULL	0	NULL	Assessment of cardiac function	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of anatomy and cardiac function by Doppler echocardiography .
	manualset3
243085	3	423806	15	NULL	NULL	0	NULL	Doppler echocardiography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of anatomy and cardiac function by Doppler echocardiography .
	manualset3
243086	1	423807	15	NULL	NULL	0	NULL	Assessment of brain tissue viability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of brain tissue viability in acute ischemic stroke by BOLD MRI .
	manualset3
243087	2	423807	15	NULL	NULL	0	NULL	acute ischemic stroke 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of brain tissue viability in acute ischemic stroke by BOLD MRI .
	manualset3
243088	3	423807	15	NULL	NULL	0	NULL	BOLD MRI	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of brain tissue viability in acute ischemic stroke by BOLD MRI .
	manualset3
243089	1	423808	15	NULL	NULL	0	NULL	Assessment of coronary artery stent patency	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of coronary artery stent patency by electron-beam CT .
	manualset3
243090	2	423808	15	NULL	NULL	0	NULL	electron-beam CT	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of coronary artery stent patency by electron-beam CT .
	manualset3
243091	1	423809	15	NULL	NULL	0	NULL	Electrocardiographic study	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Electrocardiographic and clinical study of ovariectomized women and natural menopause ) .
	manualset3
243092	2	423809	15	NULL	NULL	0	NULL	clinical study	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Electrocardiographic and clinical study of ovariectomized women and natural menopause ) .
	manualset3
243093	3	423809	15	NULL	NULL	0	NULL	ovariectomized women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Electrocardiographic and clinical study of ovariectomized women and natural menopause ) .
	manualset3
243094	4	423809	15	NULL	NULL	0	NULL	natural menopause 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Electrocardiographic and clinical study of ovariectomized women and natural menopause ) .
	manualset3
243095	1	423810	15	NULL	NULL	0	NULL	Assessment of impulsivity 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of impulsivity among psychiatric inpatients .
	manualset3
243096	2	423810	15	NULL	NULL	0	NULL	psychiatric inpatients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of impulsivity among psychiatric inpatients .
	manualset3
243099	1	423811	15	NULL	NULL	0	NULL	Assessment of margins	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of margins when excising ductal carcinoma in situ ( DCIS ) of the breast is difficult .
	manualset3
243101	2	423811	15	NULL	NULL	0	NULL	ductal carcinoma in situ ( DCIS )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of margins when excising ductal carcinoma in situ ( DCIS ) of the breast is difficult .
	manualset3
243103	3	423811	15	NULL	NULL	0	NULL	breast 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of margins when excising ductal carcinoma in situ ( DCIS ) of the breast is difficult .
	manualset3
243129	1	423812	15	NULL	NULL	0	NULL	Assessment of the burnt child	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of the burnt child includes airway , breathing and circulation stabilization , followed by assessment of the extent of the burn and head to toe examination .
	manualset3
243131	2	423812	15	NULL	NULL	0	NULL	airway stabilization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of the burnt child includes airway , breathing and circulation stabilization , followed by assessment of the extent of the burn and head to toe examination .
	manualset3
243134	3	423812	15	NULL	NULL	0	NULL	breathing stabilization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of the burnt child includes airway , breathing and circulation stabilization , followed by assessment of the extent of the burn and head to toe examination .
	manualset3
243135	4	423812	15	NULL	NULL	0	NULL	circulation stabilization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of the burnt child includes airway , breathing and circulation stabilization , followed by assessment of the extent of the burn and head to toe examination .
	manualset3
243136	5	423812	15	NULL	NULL	0	NULL	assessment of the extent of the burn 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of the burnt child includes airway , breathing and circulation stabilization , followed by assessment of the extent of the burn and head to toe examination .
	manualset3
243137	6	423812	15	NULL	NULL	0	NULL	head to toe examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of the burnt child includes airway , breathing and circulation stabilization , followed by assessment of the extent of the burn and head to toe examination .
	manualset3
243138	1	423813	15	NULL	NULL	NULL	NULL	Assessment of the concentration of sFAS 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Assessment of the concentration of sFAS indicated that the level of sFAS in subjects carrying the FAS-A/A genotype was significantly higher than that of those carrying the G/G genotype ( 3.90 ng mL ( -1 ) vs. 3.12 ng mL ( -1 ) , P = 0.035 ) .
	manualset3
243139	2	423813	15	NULL	NULL	0	NULL	level of sFAS 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of the concentration of sFAS indicated that the level of sFAS in subjects carrying the FAS-A/A genotype was significantly higher than that of those carrying the G/G genotype ( 3.90 ng mL ( -1 ) vs. 3.12 ng mL ( -1 ) , P = 0.035 ) .
	manualset3
243140	3	423813	15	NULL	NULL	0	NULL	subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of the concentration of sFAS indicated that the level of sFAS in subjects carrying the FAS-A/A genotype was significantly higher than that of those carrying the G/G genotype ( 3.90 ng mL ( -1 ) vs. 3.12 ng mL ( -1 ) , P = 0.035 ) .
	manualset3
243141	4	423813	15	NULL	NULL	0	NULL	FAS-A/A genotype	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of the concentration of sFAS indicated that the level of sFAS in subjects carrying the FAS-A/A genotype was significantly higher than that of those carrying the G/G genotype ( 3.90 ng mL ( -1 ) vs. 3.12 ng mL ( -1 ) , P = 0.035 ) .
	manualset3
243142	5	423813	15	NULL	NULL	0	NULL	G/G genotype	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of the concentration of sFAS indicated that the level of sFAS in subjects carrying the FAS-A/A genotype was significantly higher than that of those carrying the G/G genotype ( 3.90 ng mL ( -1 ) vs. 3.12 ng mL ( -1 ) , P = 0.035 ) .
	manualset3
243143	6	423813	15	NULL	NULL	0	NULL	3.90 ng mL ( -1 ) vs. 3.12 ng mL ( -1 ) , P = 0.035	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of the concentration of sFAS indicated that the level of sFAS in subjects carrying the FAS-A/A genotype was significantly higher than that of those carrying the G/G genotype ( 3.90 ng mL ( -1 ) vs. 3.12 ng mL ( -1 ) , P = 0.035 ) .
	manualset3
243144	1	423814	15	NULL	NULL	0	NULL	Assessment of ventilation-perfusion distribution	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of ventilation-perfusion distribution by multiple inert gas elimination techniques : its application in the child .
	manualset3
243145	2	423814	15	NULL	NULL	0	NULL	multiple inert gas elimination techniques	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of ventilation-perfusion distribution by multiple inert gas elimination techniques : its application in the child .
	manualset3
243146	3	423814	15	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of ventilation-perfusion distribution by multiple inert gas elimination techniques : its application in the child .
	manualset3
243147	4	423814	15	NULL	NULL	0	NULL	child 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Assessment of ventilation-perfusion distribution by multiple inert gas elimination techniques : its application in the child .
	manualset3
243148	1	423815	15	NULL	NULL	0	NULL	Associate Degree Nursing Programs	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Associate Degree Nursing Programs accredited by the NLN 1989-90 .
	manualset3
243149	2	423815	15	NULL	NULL	0	NULL	NLN	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Associate Degree Nursing Programs accredited by the NLN 1989-90 .
	manualset3
243150	3	423815	15	NULL	NULL	0	NULL	1989-90	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Associate Degree Nursing Programs accredited by the NLN 1989-90 .
	manualset3
243151	1	423816	15	NULL	NULL	0	NULL	morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Associated with high morbidity , PD continues to pose a formidable challenge to pancreatic surgeons around the world .
	manualset3
243152	2	423816	15	NULL	NULL	0	NULL	PD	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Associated with high morbidity , PD continues to pose a formidable challenge to pancreatic surgeons around the world .
	manualset3
243153	3	423816	15	NULL	NULL	0	NULL	challenge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Associated with high morbidity , PD continues to pose a formidable challenge to pancreatic surgeons around the world .
	manualset3
243154	4	423816	15	NULL	NULL	0	NULL	pancreatic surgeons	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Associated with high morbidity , PD continues to pose a formidable challenge to pancreatic surgeons around the world .
	manualset3
243157	5	423816	15	NULL	NULL	0	NULL	world 	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Associated with high morbidity , PD continues to pose a formidable challenge to pancreatic surgeons around the world .
	manualset3
243160	1	423817	15	NULL	NULL	0	NULL	Association of endothelial dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Association of endothelial dysfunction with sulfur amino acid metabolism in chronic renal failure .
	manualset3
243161	2	423817	15	NULL	NULL	0	NULL	sulfur amino acid metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Association of endothelial dysfunction with sulfur amino acid metabolism in chronic renal failure .
	manualset3
243162	3	423817	15	NULL	NULL	0	NULL	chronic renal failure	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Association of endothelial dysfunction with sulfur amino acid metabolism in chronic renal failure .
	manualset3
243163	1	423818	15	NULL	NULL	0	NULL	Association of fulminant non-A non-B hepatitis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Association of fulminant non-A non-B hepatitis with homozygosity for HLA A1-B8-DR3 .
	manualset3
243164	2	423818	15	NULL	NULL	0	NULL	homozygosity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Association of fulminant non-A non-B hepatitis with homozygosity for HLA A1-B8-DR3 .
	manualset3
243165	3	423818	15	NULL	NULL	0	NULL	HLA A1-B8-DR3 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Association of fulminant non-A non-B hepatitis with homozygosity for HLA A1-B8-DR3 .
	manualset3
243166	1	423819	15	NULL	NULL	0	NULL	Electroencephalographic study	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Electroencephalographic study of meningeal tuberculosis in childhood and in particular of a case treated exclusively by isonlazid ) .
	manualset3
243167	2	423819	15	NULL	NULL	0	NULL	meningeal tuberculosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Electroencephalographic study of meningeal tuberculosis in childhood and in particular of a case treated exclusively by isonlazid ) .
	manualset3
243168	3	423819	15	NULL	NULL	0	NULL	childhood	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	( Electroencephalographic study of meningeal tuberculosis in childhood and in particular of a case treated exclusively by isonlazid ) .
	manualset3
243169	4	423819	15	NULL	NULL	0	NULL	case	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( Electroencephalographic study of meningeal tuberculosis in childhood and in particular of a case treated exclusively by isonlazid ) .
	manualset3
243170	5	423819	15	NULL	NULL	0	NULL	isonlazid	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Electroencephalographic study of meningeal tuberculosis in childhood and in particular of a case treated exclusively by isonlazid ) .
	manualset3
243171	1	423820	15	NULL	NULL	0	NULL	Association of hepatic veno-occlusive disease	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Association of hepatic veno-occlusive disease with interstitial pneumonitis in bone marrow transplant recipients .
	manualset3
243172	2	423820	15	NULL	NULL	0	NULL	interstitial pneumonitis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Association of hepatic veno-occlusive disease with interstitial pneumonitis in bone marrow transplant recipients .
	manualset3
243173	3	423820	15	NULL	NULL	0	NULL	bone marrow transplant recipients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Association of hepatic veno-occlusive disease with interstitial pneumonitis in bone marrow transplant recipients .
	manualset3
243174	1	423821	15	NULL	NULL	0	NULL	Association of innate immune activation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Association of innate immune activation with latent Epstein-Barr virus in active MS lesions .
	manualset3
243175	2	423821	15	NULL	NULL	NULL	NULL	latent Epstein-Barr virus 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Association of innate immune activation with latent Epstein-Barr virus in active MS lesions .
	manualset3
243176	3	423821	15	NULL	NULL	0	NULL	active MS lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Association of innate immune activation with latent Epstein-Barr virus in active MS lesions .
	manualset3
243177	1	423822	15	NULL	NULL	0	NULL	Association of mannose-binding lectin 2 gene polymorphic variants	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Association of mannose-binding lectin 2 gene polymorphic variants with susceptibility and clinical progression in systemic lupus erythematosus .
	manualset3
243178	2	423822	15	NULL	NULL	0	NULL	susceptibility	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Association of mannose-binding lectin 2 gene polymorphic variants with susceptibility and clinical progression in systemic lupus erythematosus .
	manualset3
243179	3	423822	15	NULL	NULL	0	NULL	clinical progression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Association of mannose-binding lectin 2 gene polymorphic variants with susceptibility and clinical progression in systemic lupus erythematosus .
	manualset3
243180	4	423822	15	NULL	NULL	0	NULL	systemic lupus erythematosus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Association of mannose-binding lectin 2 gene polymorphic variants with susceptibility and clinical progression in systemic lupus erythematosus .
	manualset3
243181	1	423823	15	NULL	NULL	NULL	NULL	Association of maternal interaction	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Association of maternal interaction with emotional regulation in 4 - and 9-month infants during the Still Face Paradigm .
	manualset3
243182	2	423823	15	NULL	NULL	0	NULL	 emotional regulation	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Association of maternal interaction with emotional regulation in 4 - and 9-month infants during the Still Face Paradigm .
	manualset3
243183	3	423823	15	NULL	NULL	0	NULL	4 - month infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Association of maternal interaction with emotional regulation in 4 - and 9-month infants during the Still Face Paradigm .
	manualset3
243184	4	423823	15	NULL	NULL	0	NULL	9-month infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Association of maternal interaction with emotional regulation in 4 - and 9-month infants during the Still Face Paradigm .
	manualset3
243185	5	423823	15	NULL	NULL	0	NULL	Still Face Paradigm	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Association of maternal interaction with emotional regulation in 4 - and 9-month infants during the Still Face Paradigm .
	manualset3
243474	1	423824	15	NULL	NULL	NULL	NULL	Association of BE6 with E6-AP	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Association of BE6 with E6-AP appears to be necessary but not sufficient for transformation by BE6 .
	manualset3
243475	2	423824	15	NULL	NULL	0	NULL	transformation by BE6	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Association of BE6 with E6-AP appears to be necessary but not sufficient for transformation by BE6 .
	manualset3
243476	1	423825	15	NULL	NULL	NULL	NULL	Association of leptin genetic polymorphism -2548 G/A	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Association of leptin genetic polymorphism -2548 G/A with gestational diabetes mellitus .
	manualset3
243477	2	423825	15	NULL	NULL	0	NULL	gestational diabetes mellitus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Association of leptin genetic polymorphism -2548 G/A with gestational diabetes mellitus .
	manualset3
243478	1	423826	15	NULL	NULL	NULL	NULL	Association	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Association of prescription H1 antihistamine use with obesity : results from the National Health and Nutrition Examination Survey .
	manualset3
243479	2	423826	15	NULL	NULL	0	NULL	prescription H1 antihistamine use	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Association of prescription H1 antihistamine use with obesity : results from the National Health and Nutrition Examination Survey .
	manualset3
243480	3	423826	15	NULL	NULL	0	NULL	obesity	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Association of prescription H1 antihistamine use with obesity : results from the National Health and Nutrition Examination Survey .
	manualset3
243481	4	423826	15	NULL	NULL	0	NULL	National Health and Nutrition Examination Survey 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Association of prescription H1 antihistamine use with obesity : results from the National Health and Nutrition Examination Survey .
	manualset3
243482	1	423827	15	NULL	NULL	NULL	NULL	Association of synapsin I 	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Association of synapsin I with phospholipid bilayers does not induce membrane destabilization .
	manualset3
243483	2	423827	15	NULL	NULL	0	NULL	phospholipid bilayers	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Association of synapsin I with phospholipid bilayers does not induce membrane destabilization .
	manualset3
243484	3	423827	15	NULL	NULL	0	NULL	membrane destabilization 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Association of synapsin I with phospholipid bilayers does not induce membrane destabilization .
	manualset3
243485	1	423828	15	NULL	NULL	0	NULL	Association Notice	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Association Notice : Ophthalmic group committee .
	manualset3
243486	2	423828	15	NULL	NULL	0	NULL	Ophthalmic group committee	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Association Notice : Ophthalmic group committee .
	manualset3
243487	1	423829	15	NULL	NULL	NULL	NULL	Association 	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Association between 1425G/A SNP in PRKCH and ischemic stroke among Chinese and Japanese populations : a meta-analysis including 3686 cases and 4589 controls .
	manualset3
243488	2	423829	15	NULL	NULL	0	NULL	1425G/A SNP in PRKCH	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Association between 1425G/A SNP in PRKCH and ischemic stroke among Chinese and Japanese populations : a meta-analysis including 3686 cases and 4589 controls .
	manualset3
243489	3	423829	15	NULL	NULL	0	NULL	1425G/A SNP in ischemic stroke	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Association between 1425G/A SNP in PRKCH and ischemic stroke among Chinese and Japanese populations : a meta-analysis including 3686 cases and 4589 controls .
	manualset3
243490	4	423829	15	NULL	NULL	0	NULL	Chinese populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Association between 1425G/A SNP in PRKCH and ischemic stroke among Chinese and Japanese populations : a meta-analysis including 3686 cases and 4589 controls .
	manualset3
243491	5	423829	15	NULL	NULL	0	NULL	Japanese populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Association between 1425G/A SNP in PRKCH and ischemic stroke among Chinese and Japanese populations : a meta-analysis including 3686 cases and 4589 controls .
	manualset3
243492	6	423829	15	NULL	NULL	0	NULL	meta-analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Association between 1425G/A SNP in PRKCH and ischemic stroke among Chinese and Japanese populations : a meta-analysis including 3686 cases and 4589 controls .
	manualset3
243493	7	423829	15	NULL	NULL	0	NULL	3686 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Association between 1425G/A SNP in PRKCH and ischemic stroke among Chinese and Japanese populations : a meta-analysis including 3686 cases and 4589 controls .
	manualset3
243494	8	423829	15	NULL	NULL	0	NULL	4589 controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Association between 1425G/A SNP in PRKCH and ischemic stroke among Chinese and Japanese populations : a meta-analysis including 3686 cases and 4589 controls .
	manualset3
243495	1	423830	15	NULL	NULL	NULL	NULL	Association	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Association between estrogen receptor alpha polymorphisms and equol production , and its relation to bone mass .
	manualset3
243496	3	423830	15	NULL	NULL	NULL	NULL	equol production	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Association between estrogen receptor alpha polymorphisms and equol production , and its relation to bone mass .
	manualset3
243497	4	423830	15	NULL	NULL	NULL	NULL	relation	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Association between estrogen receptor alpha polymorphisms and equol production , and its relation to bone mass .
	manualset3
243498	5	423830	15	NULL	NULL	NULL	NULL	bone mass	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Association between estrogen receptor alpha polymorphisms and equol production , and its relation to bone mass .
	manualset3
243499	2	423830	15	NULL	NULL	0	NULL	estrogen receptor alpha polymorphisms 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Association between estrogen receptor alpha polymorphisms and equol production , and its relation to bone mass .
	manualset3
243500	1	423831	15	NULL	NULL	0	NULL	Association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Association between low functional health literacy and mortality in older adults : longitudinal cohort study .
	manualset3
243501	2	423831	15	NULL	NULL	0	NULL	functional health literacy	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Association between low functional health literacy and mortality in older adults : longitudinal cohort study .
	manualset3
243502	3	423831	15	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Association between low functional health literacy and mortality in older adults : longitudinal cohort study .
	manualset3
243503	4	423831	15	NULL	NULL	0	NULL	older adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Association between low functional health literacy and mortality in older adults : longitudinal cohort study .
	manualset3
243504	5	423831	15	NULL	NULL	0	NULL	longitudinal cohort study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Association between low functional health literacy and mortality in older adults : longitudinal cohort study .
	manualset3
243505	1	423832	15	NULL	NULL	NULL	NULL	Association 	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Association between the defective Pro369Ser mutation and in vivo intrahepatic 1-antitrypsin accumulation .
	manualset3
243506	2	423832	15	NULL	NULL	0	NULL	Pro369Ser mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Association between the defective Pro369Ser mutation and in vivo intrahepatic 1-antitrypsin accumulation .
	manualset3
243507	3	423832	15	NULL	NULL	0	NULL	intrahepatic 1-antitrypsin accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Association between the defective Pro369Ser mutation and in vivo intrahepatic 1-antitrypsin accumulation .
	manualset3
243508	1	423833	15	NULL	NULL	0	NULL	Association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Association between the oxytocin receptor gene and amygdalar volume in healthy adults .
	manualset3
243509	2	423833	15	NULL	NULL	0	NULL	oxytocin receptor gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Association between the oxytocin receptor gene and amygdalar volume in healthy adults .
	manualset3
243510	3	423833	15	NULL	NULL	0	NULL	amygdalar volume	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Association between the oxytocin receptor gene and amygdalar volume in healthy adults .
	manualset3
243511	4	423833	15	NULL	NULL	0	NULL	healthy adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Association between the oxytocin receptor gene and amygdalar volume in healthy adults .
	manualset3
243512	1	423834	15	NULL	NULL	0	NULL	Associations 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Associations between academic achievement and the remaining sleep variables as well as the academic , well-being , and lifestyle variables lost significance in stepwise regression .
	manualset3
243513	2	423834	15	NULL	NULL	0	NULL	academic achievement 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Associations between academic achievement and the remaining sleep variables as well as the academic , well-being , and lifestyle variables lost significance in stepwise regression .
	manualset3
243514	3	423834	15	NULL	NULL	0	NULL	sleep variables	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Associations between academic achievement and the remaining sleep variables as well as the academic , well-being , and lifestyle variables lost significance in stepwise regression .
	manualset3
243515	4	423834	15	NULL	NULL	0	NULL	academic variables	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Associations between academic achievement and the remaining sleep variables as well as the academic , well-being , and lifestyle variables lost significance in stepwise regression .
	manualset3
243516	5	423834	15	NULL	NULL	0	NULL	well-being variables	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Associations between academic achievement and the remaining sleep variables as well as the academic , well-being , and lifestyle variables lost significance in stepwise regression .
	manualset3
243517	6	423834	15	NULL	NULL	0	NULL	lifestyle variables 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Associations between academic achievement and the remaining sleep variables as well as the academic , well-being , and lifestyle variables lost significance in stepwise regression .
	manualset3
243518	7	423834	15	NULL	NULL	0	NULL	significance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Associations between academic achievement and the remaining sleep variables as well as the academic , well-being , and lifestyle variables lost significance in stepwise regression .
	manualset3
243519	8	423834	15	NULL	NULL	0	NULL	stepwise regression	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Associations between academic achievement and the remaining sleep variables as well as the academic , well-being , and lifestyle variables lost significance in stepwise regression .
	manualset3
243520	1	423835	15	NULL	NULL	0	NULL	Associations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Associations between novel single nucleotide polymorphisms in the Bos taurus growth hormone gene and performance traits in Holstein-Friesian dairy cattle .
	manualset3
243521	2	423835	15	NULL	NULL	0	NULL	single nucleotide polymorphisms	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Associations between novel single nucleotide polymorphisms in the Bos taurus growth hormone gene and performance traits in Holstein-Friesian dairy cattle .
	manualset3
243522	3	423835	15	NULL	NULL	0	NULL	Bos taurus growth hormone gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Associations between novel single nucleotide polymorphisms in the Bos taurus growth hormone gene and performance traits in Holstein-Friesian dairy cattle .
	manualset3
243523	4	423835	15	NULL	NULL	0	NULL	performance traits	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Associations between novel single nucleotide polymorphisms in the Bos taurus growth hormone gene and performance traits in Holstein-Friesian dairy cattle .
	manualset3
243524	5	423835	15	NULL	NULL	0	NULL	Holstein-Friesian dairy cattle	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Associations between novel single nucleotide polymorphisms in the Bos taurus growth hormone gene and performance traits in Holstein-Friesian dairy cattle .
	manualset3
243525	1	423836	15	NULL	NULL	NULL	NULL	initial provider cost of angioplasty	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Assume that the initial provider cost of angioplasty is $ 12 , 000 and that restenosis within 6 months results in repeat angioplasty in 20 % of cases , with a follow-up cost of $ 2 , 400 , or $ 14 , 400 total .
	manualset3
243526	2	423836	15	NULL	NULL	0	NULL	$ 12 , 000 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Assume that the initial provider cost of angioplasty is $ 12 , 000 and that restenosis within 6 months results in repeat angioplasty in 20 % of cases , with a follow-up cost of $ 2 , 400 , or $ 14 , 400 total .
	manualset3
243527	3	423836	15	NULL	NULL	0	NULL	restenosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Assume that the initial provider cost of angioplasty is $ 12 , 000 and that restenosis within 6 months results in repeat angioplasty in 20 % of cases , with a follow-up cost of $ 2 , 400 , or $ 14 , 400 total .
	manualset3
243528	4	423836	15	NULL	NULL	0	NULL	6 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Assume that the initial provider cost of angioplasty is $ 12 , 000 and that restenosis within 6 months results in repeat angioplasty in 20 % of cases , with a follow-up cost of $ 2 , 400 , or $ 14 , 400 total .
	manualset3
243529	5	423836	15	NULL	NULL	0	NULL	repeat angioplasty	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Assume that the initial provider cost of angioplasty is $ 12 , 000 and that restenosis within 6 months results in repeat angioplasty in 20 % of cases , with a follow-up cost of $ 2 , 400 , or $ 14 , 400 total .
	manualset3
243530	6	423836	15	NULL	NULL	0	NULL	20 % of cases 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Assume that the initial provider cost of angioplasty is $ 12 , 000 and that restenosis within 6 months results in repeat angioplasty in 20 % of cases , with a follow-up cost of $ 2 , 400 , or $ 14 , 400 total .
	manualset3
243531	7	423836	15	NULL	NULL	NULL	NULL	follow-up cost	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Assume that the initial provider cost of angioplasty is $ 12 , 000 and that restenosis within 6 months results in repeat angioplasty in 20 % of cases , with a follow-up cost of $ 2 , 400 , or $ 14 , 400 total .
	manualset3
243532	8	423836	15	NULL	NULL	0	NULL	$ 2 , 400 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Assume that the initial provider cost of angioplasty is $ 12 , 000 and that restenosis within 6 months results in repeat angioplasty in 20 % of cases , with a follow-up cost of $ 2 , 400 , or $ 14 , 400 total .
	manualset3
243533	9	423836	15	NULL	NULL	0	NULL	$ 14 , 400	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Assume that the initial provider cost of angioplasty is $ 12 , 000 and that restenosis within 6 months results in repeat angioplasty in 20 % of cases , with a follow-up cost of $ 2 , 400 , or $ 14 , 400 total .
	manualset3
243534	1	423837	15	NULL	NULL	0	NULL	sensitivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Assuming a sensitivity of the PCR-ELISA on night blood of 100 % , the sensitivity of night blood filtration is 74 % and that of the PCR-ELISA on day blood is 68 % .
	manualset3
243535	2	423837	15	NULL	NULL	0	NULL	PCR-ELISA 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Assuming a sensitivity of the PCR-ELISA on night blood of 100 % , the sensitivity of night blood filtration is 74 % and that of the PCR-ELISA on day blood is 68 % .
	manualset3
243536	3	423837	15	NULL	NULL	0	NULL	night blood of 100 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Assuming a sensitivity of the PCR-ELISA on night blood of 100 % , the sensitivity of night blood filtration is 74 % and that of the PCR-ELISA on day blood is 68 % .
	manualset3
243537	4	423837	15	NULL	NULL	0	NULL	sensitivity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Assuming a sensitivity of the PCR-ELISA on night blood of 100 % , the sensitivity of night blood filtration is 74 % and that of the PCR-ELISA on day blood is 68 % .
	manualset3
243538	5	423837	15	NULL	NULL	0	NULL	night blood filtration is 74 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Assuming a sensitivity of the PCR-ELISA on night blood of 100 % , the sensitivity of night blood filtration is 74 % and that of the PCR-ELISA on day blood is 68 % .
	manualset3
243539	6	423837	15	NULL	NULL	0	NULL	PCR-ELISA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Assuming a sensitivity of the PCR-ELISA on night blood of 100 % , the sensitivity of night blood filtration is 74 % and that of the PCR-ELISA on day blood is 68 % .
	manualset3
243540	7	423837	15	NULL	NULL	0	NULL	day blood is 68 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Assuming a sensitivity of the PCR-ELISA on night blood of 100 % , the sensitivity of night blood filtration is 74 % and that of the PCR-ELISA on day blood is 68 % .
	manualset3
243541	1	423838	15	NULL	NULL	0	NULL	Electrophysiological changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Electrophysiological changes in the state of uterine muscles under the action of agents stimulating histamine H1 and H2 receptors ) .
	manualset3
243542	2	423838	15	NULL	NULL	0	NULL	state of uterine muscles	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Electrophysiological changes in the state of uterine muscles under the action of agents stimulating histamine H1 and H2 receptors ) .
	manualset3
243543	3	423838	15	NULL	NULL	0	NULL	action of agents	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Electrophysiological changes in the state of uterine muscles under the action of agents stimulating histamine H1 and H2 receptors ) .
	manualset3
243544	4	423838	15	NULL	NULL	0	NULL	histamine H1 receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Electrophysiological changes in the state of uterine muscles under the action of agents stimulating histamine H1 and H2 receptors ) .
	manualset3
243545	5	423838	15	NULL	NULL	0	NULL	H2 receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Electrophysiological changes in the state of uterine muscles under the action of agents stimulating histamine H1 and H2 receptors ) .
	manualset3
243546	1	423839	15	NULL	NULL	0	NULL	larval settlement	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Assuming larval settlement occurred following entanglement , barnacle growth-rate data suggest the rope had been around the shark for at least 150 days .
	manualset3
243547	2	423839	15	NULL	NULL	0	NULL	entanglement	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Assuming larval settlement occurred following entanglement , barnacle growth-rate data suggest the rope had been around the shark for at least 150 days .
	manualset3
243548	3	423839	15	NULL	NULL	0	NULL	barnacle growth-rate data 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Assuming larval settlement occurred following entanglement , barnacle growth-rate data suggest the rope had been around the shark for at least 150 days .
	manualset3
243549	4	423839	15	NULL	NULL	0	NULL	rope	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Assuming larval settlement occurred following entanglement , barnacle growth-rate data suggest the rope had been around the shark for at least 150 days .
	manualset3
243550	5	423839	15	NULL	NULL	0	NULL	shark	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Assuming larval settlement occurred following entanglement , barnacle growth-rate data suggest the rope had been around the shark for at least 150 days .
	manualset3
243551	6	423839	15	NULL	NULL	0	NULL	150 days	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Assuming larval settlement occurred following entanglement , barnacle growth-rate data suggest the rope had been around the shark for at least 150 days .
	manualset3
243552	1	423840	15	NULL	NULL	0	NULL	serum-to-saliva transfer of insulin	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Assuming that the serum-to-saliva transfer of insulin reflects internalization and re-cycling of the hormone in the membrane-located binding sites of salivary epithelial cells and that these cells have in obesity a ` marked decrease in insulin receptor content , it has been postulated that insulin resistance in infantile obesity can be detected by the changes in the salivary immunoreactive insulin during the oral glucose tolerance test ( OGTT ) .
	manualset3
243553	2	423840	15	NULL	NULL	NULL	NULL	internalization of the hormone	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Assuming that the serum-to-saliva transfer of insulin reflects internalization and re-cycling of the hormone in the membrane-located binding sites of salivary epithelial cells and that these cells have in obesity a ` marked decrease in insulin receptor content , it has been postulated that insulin resistance in infantile obesity can be detected by the changes in the salivary immunoreactive insulin during the oral glucose tolerance test ( OGTT ) .
	manualset3
243554	3	423840	15	NULL	NULL	0	NULL	re-cycling of the hormone	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Assuming that the serum-to-saliva transfer of insulin reflects internalization and re-cycling of the hormone in the membrane-located binding sites of salivary epithelial cells and that these cells have in obesity a ` marked decrease in insulin receptor content , it has been postulated that insulin resistance in infantile obesity can be detected by the changes in the salivary immunoreactive insulin during the oral glucose tolerance test ( OGTT ) .
	manualset3
243555	4	423840	15	NULL	NULL	0	NULL	membrane-located binding sites of salivary epithelial cells	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Assuming that the serum-to-saliva transfer of insulin reflects internalization and re-cycling of the hormone in the membrane-located binding sites of salivary epithelial cells and that these cells have in obesity a ` marked decrease in insulin receptor content , it has been postulated that insulin resistance in infantile obesity can be detected by the changes in the salivary immunoreactive insulin during the oral glucose tolerance test ( OGTT ) .
	manualset3
243556	5	423840	15	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Assuming that the serum-to-saliva transfer of insulin reflects internalization and re-cycling of the hormone in the membrane-located binding sites of salivary epithelial cells and that these cells have in obesity a ` marked decrease in insulin receptor content , it has been postulated that insulin resistance in infantile obesity can be detected by the changes in the salivary immunoreactive insulin during the oral glucose tolerance test ( OGTT ) .
	manualset3
243557	6	423840	15	NULL	NULL	0	NULL	obesity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Assuming that the serum-to-saliva transfer of insulin reflects internalization and re-cycling of the hormone in the membrane-located binding sites of salivary epithelial cells and that these cells have in obesity a ` marked decrease in insulin receptor content , it has been postulated that insulin resistance in infantile obesity can be detected by the changes in the salivary immunoreactive insulin during the oral glucose tolerance test ( OGTT ) .
	manualset3
243558	7	423840	15	NULL	NULL	0	NULL	 marked decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Assuming that the serum-to-saliva transfer of insulin reflects internalization and re-cycling of the hormone in the membrane-located binding sites of salivary epithelial cells and that these cells have in obesity a ` marked decrease in insulin receptor content , it has been postulated that insulin resistance in infantile obesity can be detected by the changes in the salivary immunoreactive insulin during the oral glucose tolerance test ( OGTT ) .
	manualset3
243559	8	423840	15	NULL	NULL	0	NULL	insulin receptor content	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Assuming that the serum-to-saliva transfer of insulin reflects internalization and re-cycling of the hormone in the membrane-located binding sites of salivary epithelial cells and that these cells have in obesity a ` marked decrease in insulin receptor content , it has been postulated that insulin resistance in infantile obesity can be detected by the changes in the salivary immunoreactive insulin during the oral glucose tolerance test ( OGTT ) .
	manualset3
243560	9	423840	15	NULL	NULL	0	NULL	insulin resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Assuming that the serum-to-saliva transfer of insulin reflects internalization and re-cycling of the hormone in the membrane-located binding sites of salivary epithelial cells and that these cells have in obesity a ` marked decrease in insulin receptor content , it has been postulated that insulin resistance in infantile obesity can be detected by the changes in the salivary immunoreactive insulin during the oral glucose tolerance test ( OGTT ) .
	manualset3
243561	10	423840	15	NULL	NULL	0	NULL	infantile obesity	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Assuming that the serum-to-saliva transfer of insulin reflects internalization and re-cycling of the hormone in the membrane-located binding sites of salivary epithelial cells and that these cells have in obesity a ` marked decrease in insulin receptor content , it has been postulated that insulin resistance in infantile obesity can be detected by the changes in the salivary immunoreactive insulin during the oral glucose tolerance test ( OGTT ) .
	manualset3
243562	11	423840	15	NULL	NULL	0	NULL	changes in the salivary immunoreactive insulin 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Assuming that the serum-to-saliva transfer of insulin reflects internalization and re-cycling of the hormone in the membrane-located binding sites of salivary epithelial cells and that these cells have in obesity a ` marked decrease in insulin receptor content , it has been postulated that insulin resistance in infantile obesity can be detected by the changes in the salivary immunoreactive insulin during the oral glucose tolerance test ( OGTT ) .
	manualset3
243563	12	423840	15	NULL	NULL	0	NULL	oral glucose tolerance test ( OGTT )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Assuming that the serum-to-saliva transfer of insulin reflects internalization and re-cycling of the hormone in the membrane-located binding sites of salivary epithelial cells and that these cells have in obesity a ` marked decrease in insulin receptor content , it has been postulated that insulin resistance in infantile obesity can be detected by the changes in the salivary immunoreactive insulin during the oral glucose tolerance test ( OGTT ) .
	manualset3
253201	1	423841	15	NULL	NULL	0	NULL	fish safety	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Assuring fish safety and quality in international fish trade .
	manualset3
253202	2	423841	15	NULL	NULL	0	NULL	fish quality	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Assuring fish safety and quality in international fish trade .
	manualset3
253203	3	423841	15	NULL	NULL	0	NULL	international fish trade	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Assuring fish safety and quality in international fish trade .
	manualset3
253461	1	423842	15	NULL	NULL	NULL	NULL	Asthma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Asthma has a major impact on the health-related quality of life in the community , comparable to other chronic diseases .
	manualset3
253462	2	423842	15	NULL	NULL	NULL	NULL	impact	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Asthma has a major impact on the health-related quality of life in the community , comparable to other chronic diseases .
	manualset3
253463	3	423842	15	NULL	NULL	NULL	NULL	quality of life	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Asthma has a major impact on the health-related quality of life in the community , comparable to other chronic diseases .
	manualset3
253464	4	423842	15	NULL	NULL	NULL	NULL	community	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Asthma has a major impact on the health-related quality of life in the community , comparable to other chronic diseases .
	manualset3
253465	5	423842	15	NULL	NULL	NULL	NULL	chronic diseases	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Asthma has a major impact on the health-related quality of life in the community , comparable to other chronic diseases .
	manualset3
253466	1	423843	15	NULL	NULL	NULL	NULL	Asthma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Asthma is a chronic inflammatory disorder of airways that affects approximately 300 million adults and children worldwide .
	manualset3
253467	2	423843	15	NULL	NULL	NULL	NULL	chronic inflammatory disorder	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Asthma is a chronic inflammatory disorder of airways that affects approximately 300 million adults and children worldwide .
	manualset3
253468	3	423843	15	NULL	NULL	NULL	NULL	airways	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Asthma is a chronic inflammatory disorder of airways that affects approximately 300 million adults and children worldwide .
	manualset3
253469	4	423843	15	NULL	NULL	NULL	NULL	300 million adults	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Asthma is a chronic inflammatory disorder of airways that affects approximately 300 million adults and children worldwide .
	manualset3
253470	5	423843	15	NULL	NULL	NULL	NULL	children	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Asthma is a chronic inflammatory disorder of airways that affects approximately 300 million adults and children worldwide .
	manualset3
253471	1	423844	15	NULL	NULL	NULL	NULL	Asthma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Asthma frequently commences in early life during airway and immune development and exposure to new environmental challenges .
	manualset3
253472	2	423844	15	NULL	NULL	NULL	NULL	early life	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Asthma frequently commences in early life during airway and immune development and exposure to new environmental challenges .
	manualset3
253473	3	423844	15	NULL	NULL	NULL	NULL	airway development	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Asthma frequently commences in early life during airway and immune development and exposure to new environmental challenges .
	manualset3
253474	4	423844	15	NULL	NULL	NULL	NULL	immune development	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Asthma frequently commences in early life during airway and immune development and exposure to new environmental challenges .
	manualset3
253475	5	423844	15	NULL	NULL	NULL	NULL	exposure	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Asthma frequently commences in early life during airway and immune development and exposure to new environmental challenges .
	manualset3
253476	6	423844	15	NULL	NULL	NULL	NULL	environmental challenges	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Asthma frequently commences in early life during airway and immune development and exposure to new environmental challenges .
	manualset3
253477	1	423845	15	NULL	NULL	NULL	NULL	Astral microtubule dynamics	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astral microtubule dynamics are critical to the mechanism that ensures nuclear migration to the bud neck .
	manualset3
253478	2	423845	15	NULL	NULL	NULL	NULL	mechanism	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astral microtubule dynamics are critical to the mechanism that ensures nuclear migration to the bud neck .
	manualset3
253479	3	423845	15	NULL	NULL	NULL	NULL	nuclear migration 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astral microtubule dynamics are critical to the mechanism that ensures nuclear migration to the bud neck .
	manualset3
253480	4	423845	15	NULL	NULL	NULL	NULL	bud neck	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astral microtubule dynamics are critical to the mechanism that ensures nuclear migration to the bud neck .
	manualset3
253481	1	423846	15	NULL	NULL	NULL	NULL	Elements	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Elements for standardization of BCG vaccine ) .
	manualset3
253482	2	423846	15	NULL	NULL	NULL	NULL	standardization of BCG vaccine	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Elements for standardization of BCG vaccine ) .
	manualset3
253483	1	423847	15	NULL	NULL	NULL	NULL	Astrocytes 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astrocytes adjacent to areas of parenchymal disruption caused either by the lesion or by the instrumentation procedure became reactive , as evidenced by cellular hypertrophy and up-regulation of glial fibrillary acidic protein ( GFAP ) immunolabeling .
	manualset3
253484	2	423847	15	NULL	NULL	NULL	NULL	areas of parenchymal disruption 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astrocytes adjacent to areas of parenchymal disruption caused either by the lesion or by the instrumentation procedure became reactive , as evidenced by cellular hypertrophy and up-regulation of glial fibrillary acidic protein ( GFAP ) immunolabeling .
	manualset3
253485	3	423847	15	NULL	NULL	NULL	NULL	lesion	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astrocytes adjacent to areas of parenchymal disruption caused either by the lesion or by the instrumentation procedure became reactive , as evidenced by cellular hypertrophy and up-regulation of glial fibrillary acidic protein ( GFAP ) immunolabeling .
	manualset3
253486	4	423847	15	NULL	NULL	NULL	NULL	instrumentation procedure	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astrocytes adjacent to areas of parenchymal disruption caused either by the lesion or by the instrumentation procedure became reactive , as evidenced by cellular hypertrophy and up-regulation of glial fibrillary acidic protein ( GFAP ) immunolabeling .
	manualset3
253487	5	423847	15	NULL	NULL	NULL	NULL	cellular hypertrophy 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astrocytes adjacent to areas of parenchymal disruption caused either by the lesion or by the instrumentation procedure became reactive , as evidenced by cellular hypertrophy and up-regulation of glial fibrillary acidic protein ( GFAP ) immunolabeling .
	manualset3
253488	6	423847	15	NULL	NULL	NULL	NULL	up-regulation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astrocytes adjacent to areas of parenchymal disruption caused either by the lesion or by the instrumentation procedure became reactive , as evidenced by cellular hypertrophy and up-regulation of glial fibrillary acidic protein ( GFAP ) immunolabeling .
	manualset3
253489	7	423847	15	NULL	NULL	NULL	NULL	glial fibrillary acidic protein ( GFAP ) immunolabeling	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astrocytes adjacent to areas of parenchymal disruption caused either by the lesion or by the instrumentation procedure became reactive , as evidenced by cellular hypertrophy and up-regulation of glial fibrillary acidic protein ( GFAP ) immunolabeling .
	manualset3
253490	1	423848	15	NULL	NULL	NULL	NULL	Astrocytes	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astrocytes in the barrel cortex respond with a transient Ca2 + increase to neuronal stimulation and this response is restricted to the stimulated barrel field .
	manualset3
253491	2	423848	15	NULL	NULL	NULL	NULL	barrel cortex	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astrocytes in the barrel cortex respond with a transient Ca2 + increase to neuronal stimulation and this response is restricted to the stimulated barrel field .
	manualset3
253492	3	423848	15	NULL	NULL	NULL	NULL	Ca2 +	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astrocytes in the barrel cortex respond with a transient Ca2 + increase to neuronal stimulation and this response is restricted to the stimulated barrel field .
	manualset3
253493	5	423848	15	NULL	NULL	NULL	NULL	neuronal stimulation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astrocytes in the barrel cortex respond with a transient Ca2 + increase to neuronal stimulation and this response is restricted to the stimulated barrel field .
	manualset3
253494	6	423848	15	NULL	NULL	NULL	NULL	response	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astrocytes in the barrel cortex respond with a transient Ca2 + increase to neuronal stimulation and this response is restricted to the stimulated barrel field .
	manualset3
253495	7	423848	15	NULL	NULL	NULL	NULL	barrel field 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astrocytes in the barrel cortex respond with a transient Ca2 + increase to neuronal stimulation and this response is restricted to the stimulated barrel field .
	manualset3
259591	4	423848	15	NULL	NULL	NULL	NULL	increase	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astrocytes in the barrel cortex respond with a transient Ca2 + increase to neuronal stimulation and this response is restricted to the stimulated barrel field .
	manualset3
253497	1	423849	15	NULL	NULL	NULL	NULL	Astrocytes	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astrocytes in the retinal part of ION had longer processes filled with abundant gliofilaments .
	manualset3
253498	2	423849	15	NULL	NULL	NULL	NULL	retinal part of ION	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astrocytes in the retinal part of ION had longer processes filled with abundant gliofilaments .
	manualset3
253499	3	423849	15	NULL	NULL	NULL	NULL	processes	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astrocytes in the retinal part of ION had longer processes filled with abundant gliofilaments .
	manualset3
253500	4	423849	15	NULL	NULL	NULL	NULL	gliofilaments 	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astrocytes in the retinal part of ION had longer processes filled with abundant gliofilaments .
	manualset3
253503	1	423850	15	NULL	NULL	NULL	NULL	Astrocytes	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astrocytes which became reactive after producing an artificial scar or after addition of certain compounds such as dibutyryl cyclic AMP , interleukin-6 , basic fibroblast growth factor and kainic acid , also revealed GABA ( A ) - receptor immunoreactivity .
	manualset3
253511	2	423850	15	NULL	NULL	NULL	NULL	artificial scar	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astrocytes which became reactive after producing an artificial scar or after addition of certain compounds such as dibutyryl cyclic AMP , interleukin-6 , basic fibroblast growth factor and kainic acid , also revealed GABA ( A ) - receptor immunoreactivity .
	manualset3
253514	3	423850	15	NULL	NULL	NULL	NULL	addition	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astrocytes which became reactive after producing an artificial scar or after addition of certain compounds such as dibutyryl cyclic AMP , interleukin-6 , basic fibroblast growth factor and kainic acid , also revealed GABA ( A ) - receptor immunoreactivity .
	manualset3
253518	4	423850	15	NULL	NULL	NULL	NULL	certain compounds	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astrocytes which became reactive after producing an artificial scar or after addition of certain compounds such as dibutyryl cyclic AMP , interleukin-6 , basic fibroblast growth factor and kainic acid , also revealed GABA ( A ) - receptor immunoreactivity .
	manualset3
253519	5	423850	15	NULL	NULL	NULL	NULL	dibutyryl cyclic AMP	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astrocytes which became reactive after producing an artificial scar or after addition of certain compounds such as dibutyryl cyclic AMP , interleukin-6 , basic fibroblast growth factor and kainic acid , also revealed GABA ( A ) - receptor immunoreactivity .
	manualset3
253523	6	423850	15	NULL	NULL	NULL	NULL	interleukin-6	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astrocytes which became reactive after producing an artificial scar or after addition of certain compounds such as dibutyryl cyclic AMP , interleukin-6 , basic fibroblast growth factor and kainic acid , also revealed GABA ( A ) - receptor immunoreactivity .
	manualset3
253525	7	423850	15	NULL	NULL	NULL	NULL	fibroblast growth factor	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astrocytes which became reactive after producing an artificial scar or after addition of certain compounds such as dibutyryl cyclic AMP , interleukin-6 , basic fibroblast growth factor and kainic acid , also revealed GABA ( A ) - receptor immunoreactivity .
	manualset3
253534	8	423850	15	NULL	NULL	NULL	NULL	kainic acid	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astrocytes which became reactive after producing an artificial scar or after addition of certain compounds such as dibutyryl cyclic AMP , interleukin-6 , basic fibroblast growth factor and kainic acid , also revealed GABA ( A ) - receptor immunoreactivity .
	manualset3
253535	9	423850	15	NULL	NULL	NULL	NULL	GABA ( A ) - receptor immunoreactivity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Astrocytes which became reactive after producing an artificial scar or after addition of certain compounds such as dibutyryl cyclic AMP , interleukin-6 , basic fibroblast growth factor and kainic acid , also revealed GABA ( A ) - receptor immunoreactivity .
	manualset3
253546	1	423851	15	NULL	NULL	NULL	NULL	Asymptomatic carotid artery stenting	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Asymptomatic carotid artery stenting : Filter or no filter ?
	manualset3
253548	1	423852	15	NULL	NULL	NULL	NULL	Asymptomatic gastroduodenal anisakiasis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Asymptomatic gastroduodenal anisakiasis as the cause of anaphylaxis .
	manualset3
253549	2	423852	15	NULL	NULL	NULL	NULL	anaphylaxis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Asymptomatic gastroduodenal anisakiasis as the cause of anaphylaxis .
	manualset3
253550	1	423853	15	NULL	NULL	NULL	NULL	Asymptomatic hyperammonemia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Asymptomatic hyperammonemia occurs in 15-50 % of valproate-treated patients , and while the true incidence of VHE is not known , it is a recognized complication of sodium valproate treatment .
	manualset3
253552	2	423853	15	NULL	NULL	NULL	NULL	15-50 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Asymptomatic hyperammonemia occurs in 15-50 % of valproate-treated patients , and while the true incidence of VHE is not known , it is a recognized complication of sodium valproate treatment .
	manualset3
253553	3	423853	15	NULL	NULL	NULL	NULL	valproate-treated patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Asymptomatic hyperammonemia occurs in 15-50 % of valproate-treated patients , and while the true incidence of VHE is not known , it is a recognized complication of sodium valproate treatment .
	manualset3
253554	4	423853	15	NULL	NULL	NULL	NULL	incidence 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Asymptomatic hyperammonemia occurs in 15-50 % of valproate-treated patients , and while the true incidence of VHE is not known , it is a recognized complication of sodium valproate treatment .
	manualset3
253555	5	423853	15	NULL	NULL	NULL	NULL	VHE	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Asymptomatic hyperammonemia occurs in 15-50 % of valproate-treated patients , and while the true incidence of VHE is not known , it is a recognized complication of sodium valproate treatment .
	manualset3
253556	6	423853	15	NULL	NULL	NULL	NULL	complication	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Asymptomatic hyperammonemia occurs in 15-50 % of valproate-treated patients , and while the true incidence of VHE is not known , it is a recognized complication of sodium valproate treatment .
	manualset3
253557	7	423853	15	NULL	NULL	NULL	NULL	sodium valproate treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Asymptomatic hyperammonemia occurs in 15-50 % of valproate-treated patients , and while the true incidence of VHE is not known , it is a recognized complication of sodium valproate treatment .
	manualset3
253607	1	423854	15	NULL	NULL	NULL	NULL	clinical case	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( A clinical case of chloromycetin treatment for abdominal typhus ) .
	manualset3
253609	2	423854	15	NULL	NULL	NULL	NULL	chloromycetin treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( A clinical case of chloromycetin treatment for abdominal typhus ) .
	manualset3
253610	3	423854	15	NULL	NULL	NULL	NULL	abdominal typhus	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( A clinical case of chloromycetin treatment for abdominal typhus ) .
	manualset3
253616	1	423855	15	NULL	NULL	NULL	NULL	voyage	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Endless voyage : life of Ms. Shin Tanaka .
	manualset3
253622	2	423855	15	NULL	NULL	NULL	NULL	Ms. Shin Tanaka	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Endless voyage : life of Ms. Shin Tanaka .
	manualset3
253626	1	423856	15	NULL	NULL	NULL	NULL	Asymptomatic osteonecrosis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Asymptomatic osteonecrosis : should it be treated ?
	manualset3
253627	1	423857	15	NULL	NULL	NULL	NULL	0.01 microgram/kg min-1 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 0.01 microgram/kg min-1 prostacyclin had no effect on blood pressure in normotensive sheep or on the development of ACTH hypertension .
	manualset3
253628	2	423857	15	NULL	NULL	NULL	NULL	prostacyclin	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 0.01 microgram/kg min-1 prostacyclin had no effect on blood pressure in normotensive sheep or on the development of ACTH hypertension .
	manualset3
253629	3	423857	15	NULL	NULL	NULL	NULL	blood pressure	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 0.01 microgram/kg min-1 prostacyclin had no effect on blood pressure in normotensive sheep or on the development of ACTH hypertension .
	manualset3
253630	4	423857	15	NULL	NULL	NULL	NULL	normotensive sheep	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 0.01 microgram/kg min-1 prostacyclin had no effect on blood pressure in normotensive sheep or on the development of ACTH hypertension .
	manualset3
253631	5	423857	15	NULL	NULL	NULL	NULL	development of ACTH hypertension	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 0.01 microgram/kg min-1 prostacyclin had no effect on blood pressure in normotensive sheep or on the development of ACTH hypertension .
	manualset3
253679	1	423858	15	NULL	NULL	NULL	NULL	1.8 mM	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 1.8 mM Ca2 + in the medium this implies the necessity of an extrusion pump in the plasma membrane .
	manualset3
253680	2	423858	15	NULL	NULL	NULL	NULL	Ca2 +	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 1.8 mM Ca2 + in the medium this implies the necessity of an extrusion pump in the plasma membrane .
	manualset3
253692	3	423858	15	NULL	NULL	NULL	NULL	medium	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 1.8 mM Ca2 + in the medium this implies the necessity of an extrusion pump in the plasma membrane .
	manualset3
253696	4	423858	15	NULL	NULL	NULL	NULL	necessity	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 1.8 mM Ca2 + in the medium this implies the necessity of an extrusion pump in the plasma membrane .
	manualset3
253697	5	423858	15	NULL	NULL	NULL	NULL	extrusion pump 	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 1.8 mM Ca2 + in the medium this implies the necessity of an extrusion pump in the plasma membrane .
	manualset3
253698	6	423858	15	NULL	NULL	NULL	NULL	plasma membrane	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 1.8 mM Ca2 + in the medium this implies the necessity of an extrusion pump in the plasma membrane .
	manualset3
253699	1	423859	15	NULL	NULL	NULL	NULL	10 DPI	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 10 DPI , sexual stages were detected in the intestine from the duodenal loop through Meckel 's diverticulum but not in other organs .
	manualset3
253700	2	423859	15	NULL	NULL	NULL	NULL	sexual stages	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 10 DPI , sexual stages were detected in the intestine from the duodenal loop through Meckel 's diverticulum but not in other organs .
	manualset3
253701	3	423859	15	NULL	NULL	NULL	NULL	intestine	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 10 DPI , sexual stages were detected in the intestine from the duodenal loop through Meckel 's diverticulum but not in other organs .
	manualset3
253702	4	423859	15	NULL	NULL	NULL	NULL	duodenal loop	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 10 DPI , sexual stages were detected in the intestine from the duodenal loop through Meckel 's diverticulum but not in other organs .
	manualset3
253703	5	423859	15	NULL	NULL	NULL	NULL	Meckel 's diverticulum	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 10 DPI , sexual stages were detected in the intestine from the duodenal loop through Meckel 's diverticulum but not in other organs .
	manualset3
253704	6	423859	15	NULL	NULL	NULL	NULL	organs	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 10 DPI , sexual stages were detected in the intestine from the duodenal loop through Meckel 's diverticulum but not in other organs .
	manualset3
253705	1	423860	15	NULL	NULL	NULL	NULL	12 days after infection	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 12 days after infection , DSCG significantly reduced the severity of anaphylactic bronchoconstriction , suggesting that IgE competes with IgG1 antibody for sensitisation sites in the lung .
	manualset3
253706	2	423860	15	NULL	NULL	NULL	NULL	DSCG	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 12 days after infection , DSCG significantly reduced the severity of anaphylactic bronchoconstriction , suggesting that IgE competes with IgG1 antibody for sensitisation sites in the lung .
	manualset3
253707	3	423860	15	NULL	NULL	NULL	NULL	severity of anaphylactic bronchoconstriction	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 12 days after infection , DSCG significantly reduced the severity of anaphylactic bronchoconstriction , suggesting that IgE competes with IgG1 antibody for sensitisation sites in the lung .
	manualset3
253708	4	423860	15	NULL	NULL	NULL	NULL	IgE antibody	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 12 days after infection , DSCG significantly reduced the severity of anaphylactic bronchoconstriction , suggesting that IgE competes with IgG1 antibody for sensitisation sites in the lung .
	manualset3
253709	5	423860	15	NULL	NULL	NULL	NULL	IgG1 antibody	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 12 days after infection , DSCG significantly reduced the severity of anaphylactic bronchoconstriction , suggesting that IgE competes with IgG1 antibody for sensitisation sites in the lung .
	manualset3
253710	6	423860	15	NULL	NULL	NULL	NULL	sensitisation sites in the lung	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 12 days after infection , DSCG significantly reduced the severity of anaphylactic bronchoconstriction , suggesting that IgE competes with IgG1 antibody for sensitisation sites in the lung .
	manualset3
253711	1	423861	15	NULL	NULL	NULL	NULL	12 months	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 12 months , the LBM values were significantly correlated to the IGF-I levels ( r = 0.718 ; P & lt ; 0.001 ) , but not to ALS or IGFBP-3 levels .
	manualset3
253712	2	423861	15	NULL	NULL	NULL	NULL	LBM values	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 12 months , the LBM values were significantly correlated to the IGF-I levels ( r = 0.718 ; P & lt ; 0.001 ) , but not to ALS or IGFBP-3 levels .
	manualset3
253713	3	423861	15	NULL	NULL	NULL	NULL	IGF-I levels 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 12 months , the LBM values were significantly correlated to the IGF-I levels ( r = 0.718 ; P & lt ; 0.001 ) , but not to ALS or IGFBP-3 levels .
	manualset3
253714	4	423861	15	NULL	NULL	NULL	NULL	r = 0.718 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 12 months , the LBM values were significantly correlated to the IGF-I levels ( r = 0.718 ; P & lt ; 0.001 ) , but not to ALS or IGFBP-3 levels .
	manualset3
253715	5	423861	15	NULL	NULL	NULL	NULL	P & lt ; 0.001	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 12 months , the LBM values were significantly correlated to the IGF-I levels ( r = 0.718 ; P & lt ; 0.001 ) , but not to ALS or IGFBP-3 levels .
	manualset3
253716	6	423861	15	NULL	NULL	NULL	NULL	ALS levels	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 12 months , the LBM values were significantly correlated to the IGF-I levels ( r = 0.718 ; P & lt ; 0.001 ) , but not to ALS or IGFBP-3 levels .
	manualset3
253717	7	423861	15	NULL	NULL	NULL	NULL	IGFBP-3 levels	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 12 months , the LBM values were significantly correlated to the IGF-I levels ( r = 0.718 ; P & lt ; 0.001 ) , but not to ALS or IGFBP-3 levels .
	manualset3
253718	1	423862	15	NULL	NULL	NULL	NULL	1500 K	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 1500 K , the cobalt-carbon chemical bonds keep breaking and re-forming , providing a direct incorporation process for additional carbon , necessary for growth .
	manualset3
253719	2	423862	15	NULL	NULL	NULL	NULL	cobalt-carbon chemical bonds	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 1500 K , the cobalt-carbon chemical bonds keep breaking and re-forming , providing a direct incorporation process for additional carbon , necessary for growth .
	manualset3
253720	3	423862	15	NULL	NULL	NULL	NULL	direct incorporation process	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 1500 K , the cobalt-carbon chemical bonds keep breaking and re-forming , providing a direct incorporation process for additional carbon , necessary for growth .
	manualset3
253721	4	423862	15	NULL	NULL	NULL	NULL	carbon	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 1500 K , the cobalt-carbon chemical bonds keep breaking and re-forming , providing a direct incorporation process for additional carbon , necessary for growth .
	manualset3
253722	5	423862	15	NULL	NULL	NULL	NULL	growth	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 1500 K , the cobalt-carbon chemical bonds keep breaking and re-forming , providing a direct incorporation process for additional carbon , necessary for growth .
	manualset3
253835	1	423863	15	NULL	NULL	NULL	NULL	Endocrine data	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Endocrine data in cryptorchism ) .
	manualset3
253840	2	423863	15	NULL	NULL	NULL	NULL	cryptorchism	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Endocrine data in cryptorchism ) .
	manualset3
253841	1	423864	15	NULL	NULL	NULL	NULL	24h	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 24 , 48 , and 168h , fish were sacrificed and liver mRNA was extracted for gene expression analysis ( 24 and 168h only ) .
	manualset3
253843	2	423864	15	NULL	NULL	NULL	NULL	48h	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 24 , 48 , and 168h , fish were sacrificed and liver mRNA was extracted for gene expression analysis ( 24 and 168h only ) .
	manualset3
253845	3	423864	15	NULL	NULL	NULL	NULL	168h	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 24 , 48 , and 168h , fish were sacrificed and liver mRNA was extracted for gene expression analysis ( 24 and 168h only ) .
	manualset3
253847	4	423864	15	NULL	NULL	NULL	NULL	fish	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 24 , 48 , and 168h , fish were sacrificed and liver mRNA was extracted for gene expression analysis ( 24 and 168h only ) .
	manualset3
253860	5	423864	15	NULL	NULL	NULL	NULL	liver mRNA	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 24 , 48 , and 168h , fish were sacrificed and liver mRNA was extracted for gene expression analysis ( 24 and 168h only ) .
	manualset3
253861	6	423864	15	NULL	NULL	NULL	NULL	gene expression analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 24 , 48 , and 168h , fish were sacrificed and liver mRNA was extracted for gene expression analysis ( 24 and 168h only ) .
	manualset3
253862	7	423864	15	NULL	NULL	NULL	NULL	24h	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 24 , 48 , and 168h , fish were sacrificed and liver mRNA was extracted for gene expression analysis ( 24 and 168h only ) .
	manualset3
253863	8	423864	15	NULL	NULL	NULL	NULL	168h	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 24 , 48 , and 168h , fish were sacrificed and liver mRNA was extracted for gene expression analysis ( 24 and 168h only ) .
	manualset3
253864	1	423865	15	NULL	NULL	NULL	NULL	24 hr	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 24 hr , the T/M ratio was 0.62 + / - 0.18 .
	manualset3
253865	2	423865	15	NULL	NULL	NULL	NULL	T/M ratio	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 24 hr , the T/M ratio was 0.62 + / - 0.18 .
	manualset3
253866	3	423865	15	NULL	NULL	NULL	NULL	 0.62 + / - 0.18 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 24 hr , the T/M ratio was 0.62 + / - 0.18 .
	manualset3
253867	1	423866	15	NULL	NULL	NULL	NULL	3-4 weeks of age	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 3-4 , 15 and 26 weeks of age , oral glucose tolerance tests were performed , and pancreas tissue was collected for electron microscopy , enzyme activity assays and islet isolation .
	manualset3
253868	2	423866	15	NULL	NULL	NULL	NULL	15 weeks of age	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 3-4 , 15 and 26 weeks of age , oral glucose tolerance tests were performed , and pancreas tissue was collected for electron microscopy , enzyme activity assays and islet isolation .
	manualset3
253869	3	423866	15	NULL	NULL	NULL	NULL	26 weeks of age	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 3-4 , 15 and 26 weeks of age , oral glucose tolerance tests were performed , and pancreas tissue was collected for electron microscopy , enzyme activity assays and islet isolation .
	manualset3
253870	4	423866	15	NULL	NULL	NULL	NULL	oral glucose tolerance tests 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 3-4 , 15 and 26 weeks of age , oral glucose tolerance tests were performed , and pancreas tissue was collected for electron microscopy , enzyme activity assays and islet isolation .
	manualset3
253871	5	423866	15	NULL	NULL	NULL	NULL	pancreas tissue	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 3-4 , 15 and 26 weeks of age , oral glucose tolerance tests were performed , and pancreas tissue was collected for electron microscopy , enzyme activity assays and islet isolation .
	manualset3
253872	6	423866	15	NULL	NULL	NULL	NULL	electron microscopy	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 3-4 , 15 and 26 weeks of age , oral glucose tolerance tests were performed , and pancreas tissue was collected for electron microscopy , enzyme activity assays and islet isolation .
	manualset3
253873	7	423866	15	NULL	NULL	NULL	NULL	enzyme activity assays	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 3-4 , 15 and 26 weeks of age , oral glucose tolerance tests were performed , and pancreas tissue was collected for electron microscopy , enzyme activity assays and islet isolation .
	manualset3
253874	8	423866	15	NULL	NULL	NULL	NULL	islet isolation	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 3-4 , 15 and 26 weeks of age , oral glucose tolerance tests were performed , and pancreas tissue was collected for electron microscopy , enzyme activity assays and islet isolation .
	manualset3
253876	1	423867	15	NULL	NULL	NULL	NULL	3 weeks after implantation	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 3 weeks after implantation , the BMP-treated implants in the 2 lower dose groups had significantly more bone ingrowth to the implant surface than did the control groups , and the greatest effect occurred in the 30-g rhBMP-2 group animals .
	manualset3
253879	2	423867	15	NULL	NULL	NULL	NULL	BMP-treated implants 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 3 weeks after implantation , the BMP-treated implants in the 2 lower dose groups had significantly more bone ingrowth to the implant surface than did the control groups , and the greatest effect occurred in the 30-g rhBMP-2 group animals .
	manualset3
253885	3	423867	15	NULL	NULL	NULL	NULL	2 lower dose groups	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 3 weeks after implantation , the BMP-treated implants in the 2 lower dose groups had significantly more bone ingrowth to the implant surface than did the control groups , and the greatest effect occurred in the 30-g rhBMP-2 group animals .
	manualset3
253891	4	423867	15	NULL	NULL	NULL	NULL	bone ingrowth	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 3 weeks after implantation , the BMP-treated implants in the 2 lower dose groups had significantly more bone ingrowth to the implant surface than did the control groups , and the greatest effect occurred in the 30-g rhBMP-2 group animals .
	manualset3
253895	5	423867	15	NULL	NULL	NULL	NULL	implant surface	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 3 weeks after implantation , the BMP-treated implants in the 2 lower dose groups had significantly more bone ingrowth to the implant surface than did the control groups , and the greatest effect occurred in the 30-g rhBMP-2 group animals .
	manualset3
253897	6	423867	15	NULL	NULL	NULL	NULL	control groups	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 3 weeks after implantation , the BMP-treated implants in the 2 lower dose groups had significantly more bone ingrowth to the implant surface than did the control groups , and the greatest effect occurred in the 30-g rhBMP-2 group animals .
	manualset3
253900	7	423867	15	NULL	NULL	NULL	NULL	effect	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 3 weeks after implantation , the BMP-treated implants in the 2 lower dose groups had significantly more bone ingrowth to the implant surface than did the control groups , and the greatest effect occurred in the 30-g rhBMP-2 group animals .
	manualset3
253902	8	423867	15	NULL	NULL	NULL	NULL	30-g rhBMP-2 group animals 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 3 weeks after implantation , the BMP-treated implants in the 2 lower dose groups had significantly more bone ingrowth to the implant surface than did the control groups , and the greatest effect occurred in the 30-g rhBMP-2 group animals .
	manualset3
253910	1	423868	15	NULL	NULL	NULL	NULL	6 hr posttreatment	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 6 hr posttreatment the reverse was seen .
	manualset3
253912	2	423868	15	NULL	NULL	NULL	NULL	reverse	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 6 hr posttreatment the reverse was seen .
	manualset3
253917	1	423869	15	NULL	NULL	NULL	NULL	 65-75 kg	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 65-75 kg and 115 kg live weight pigs were slaughtered , and fat was taken for the HC determination .
	manualset3
253919	2	423869	15	NULL	NULL	NULL	NULL	115 kg	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 65-75 kg and 115 kg live weight pigs were slaughtered , and fat was taken for the HC determination .
	manualset3
253922	3	423869	15	NULL	NULL	NULL	NULL	live weight	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 65-75 kg and 115 kg live weight pigs were slaughtered , and fat was taken for the HC determination .
	manualset3
253924	4	423869	15	NULL	NULL	NULL	NULL	pigs	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 65-75 kg and 115 kg live weight pigs were slaughtered , and fat was taken for the HC determination .
	manualset3
253928	5	423869	15	NULL	NULL	NULL	NULL	fat	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 65-75 kg and 115 kg live weight pigs were slaughtered , and fat was taken for the HC determination .
	manualset3
253932	6	423869	15	NULL	NULL	NULL	NULL	HC determination	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 65-75 kg and 115 kg live weight pigs were slaughtered , and fat was taken for the HC determination .
	manualset3
253944	1	423870	15	NULL	NULL	NULL	NULL	Endoscopic clipping	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Endoscopic clipping of a gastric perforation after GIST resection ) .
	manualset3
253946	2	423870	15	NULL	NULL	NULL	NULL	gastric perforation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Endoscopic clipping of a gastric perforation after GIST resection ) .
	manualset3
253949	3	423870	15	NULL	NULL	NULL	NULL	GIST resection	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Endoscopic clipping of a gastric perforation after GIST resection ) .
	manualset3
253959	1	423871	15	NULL	NULL	NULL	NULL	7 days	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 7 , 14 and 21 days , regeneration of the muscle fiber and fibrosis in the interstitium were observed .
	manualset3
253962	2	423871	15	NULL	NULL	NULL	NULL	14 days	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 7 , 14 and 21 days , regeneration of the muscle fiber and fibrosis in the interstitium were observed .
	manualset3
253963	3	423871	15	NULL	NULL	NULL	NULL	21 days	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 7 , 14 and 21 days , regeneration of the muscle fiber and fibrosis in the interstitium were observed .
	manualset3
253967	4	423871	15	NULL	NULL	NULL	NULL	regeneration of the muscle fiber	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 7 , 14 and 21 days , regeneration of the muscle fiber and fibrosis in the interstitium were observed .
	manualset3
253969	5	423871	15	NULL	NULL	NULL	NULL	fibrosis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 7 , 14 and 21 days , regeneration of the muscle fiber and fibrosis in the interstitium were observed .
	manualset3
253970	6	423871	15	NULL	NULL	NULL	NULL	interstitium	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 7 , 14 and 21 days , regeneration of the muscle fiber and fibrosis in the interstitium were observed .
	manualset3
253984	1	423872	15	NULL	NULL	NULL	NULL	720K	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 720K the dimensionless figure of merit ZT reaches the state-of-the-art value of 1.53 for TAGS-75 and 1.50 for TAGS-80 and TAGS-85 samples , respectively .
	manualset3
253985	2	423872	15	NULL	NULL	NULL	NULL	dimensionless figure of merit ZT	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 720K the dimensionless figure of merit ZT reaches the state-of-the-art value of 1.53 for TAGS-75 and 1.50 for TAGS-80 and TAGS-85 samples , respectively .
	manualset3
253986	3	423872	15	NULL	NULL	NULL	NULL	state-of-the-art value of 1.53	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 720K the dimensionless figure of merit ZT reaches the state-of-the-art value of 1.53 for TAGS-75 and 1.50 for TAGS-80 and TAGS-85 samples , respectively .
	manualset3
253987	4	423872	15	NULL	NULL	NULL	NULL	TAGS-75	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 720K the dimensionless figure of merit ZT reaches the state-of-the-art value of 1.53 for TAGS-75 and 1.50 for TAGS-80 and TAGS-85 samples , respectively .
	manualset3
253988	5	423872	15	NULL	NULL	NULL	NULL	state-of-the-art value of 1.50	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 720K the dimensionless figure of merit ZT reaches the state-of-the-art value of 1.53 for TAGS-75 and 1.50 for TAGS-80 and TAGS-85 samples , respectively .
	manualset3
253989	6	423872	15	NULL	NULL	NULL	NULL	TAGS-80	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 720K the dimensionless figure of merit ZT reaches the state-of-the-art value of 1.53 for TAGS-75 and 1.50 for TAGS-80 and TAGS-85 samples , respectively .
	manualset3
253990	7	423872	15	NULL	NULL	NULL	NULL	TAGS-85 samples	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At 720K the dimensionless figure of merit ZT reaches the state-of-the-art value of 1.53 for TAGS-75 and 1.50 for TAGS-80 and TAGS-85 samples , respectively .
	manualset3
253991	1	423873	15	NULL	NULL	NULL	NULL	Time 1	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At Time 1 a mixed sample of community participants ( N = 85 ) were interviewed and completed self-report measures of depression , anxiety , and intrusive memory features .
	manualset3
253992	2	423873	15	NULL	NULL	NULL	NULL	mixed sample of community participants 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At Time 1 a mixed sample of community participants ( N = 85 ) were interviewed and completed self-report measures of depression , anxiety , and intrusive memory features .
	manualset3
253993	3	423873	15	NULL	NULL	NULL	NULL	N = 85	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At Time 1 a mixed sample of community participants ( N = 85 ) were interviewed and completed self-report measures of depression , anxiety , and intrusive memory features .
	manualset3
253994	4	423873	15	NULL	NULL	NULL	NULL	self-report measures	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At Time 1 a mixed sample of community participants ( N = 85 ) were interviewed and completed self-report measures of depression , anxiety , and intrusive memory features .
	manualset3
253995	5	423873	15	NULL	NULL	NULL	NULL	depression	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At Time 1 a mixed sample of community participants ( N = 85 ) were interviewed and completed self-report measures of depression , anxiety , and intrusive memory features .
	manualset3
253996	6	423873	15	NULL	NULL	NULL	NULL	anxiety	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At Time 1 a mixed sample of community participants ( N = 85 ) were interviewed and completed self-report measures of depression , anxiety , and intrusive memory features .
	manualset3
253997	7	423873	15	NULL	NULL	NULL	NULL	intrusive memory features	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At Time 1 a mixed sample of community participants ( N = 85 ) were interviewed and completed self-report measures of depression , anxiety , and intrusive memory features .
	manualset3
253998	1	423874	15	NULL	NULL	NULL	NULL	total incremental cost of +255.92	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At a total incremental cost of +255.92 per patient-day , care at the Hospital for Sick Children may not currently be the least expensive means of offering the Kozak protocol to Ontario children .
	manualset3
253999	2	423874	15	NULL	NULL	NULL	NULL	patient	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At a total incremental cost of +255.92 per patient-day , care at the Hospital for Sick Children may not currently be the least expensive means of offering the Kozak protocol to Ontario children .
	manualset3
254000	3	423874	15	NULL	NULL	NULL	NULL	day care	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At a total incremental cost of +255.92 per patient-day , care at the Hospital for Sick Children may not currently be the least expensive means of offering the Kozak protocol to Ontario children .
	manualset3
254001	4	423874	15	NULL	NULL	NULL	NULL	Hospital	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At a total incremental cost of +255.92 per patient-day , care at the Hospital for Sick Children may not currently be the least expensive means of offering the Kozak protocol to Ontario children .
	manualset3
254002	5	423874	15	NULL	NULL	NULL	NULL	Sick Children	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At a total incremental cost of +255.92 per patient-day , care at the Hospital for Sick Children may not currently be the least expensive means of offering the Kozak protocol to Ontario children .
	manualset3
254003	6	423874	15	NULL	NULL	NULL	NULL	means	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At a total incremental cost of +255.92 per patient-day , care at the Hospital for Sick Children may not currently be the least expensive means of offering the Kozak protocol to Ontario children .
	manualset3
254004	7	423874	15	NULL	NULL	NULL	NULL	Kozak protocol	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At a total incremental cost of +255.92 per patient-day , care at the Hospital for Sick Children may not currently be the least expensive means of offering the Kozak protocol to Ontario children .
	manualset3
254005	8	423874	15	NULL	NULL	NULL	NULL	Ontario children	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At a total incremental cost of +255.92 per patient-day , care at the Hospital for Sick Children may not currently be the least expensive means of offering the Kozak protocol to Ontario children .
	manualset3
254006	1	423875	15	NULL	NULL	NULL	NULL	admission	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At admission , the EBV deoxyribonucleic acid ( DNA ) blood level was 40 copies/g .
	manualset3
254007	2	423875	15	NULL	NULL	NULL	NULL	EBV deoxyribonucleic acid ( DNA ) blood level	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At admission , the EBV deoxyribonucleic acid ( DNA ) blood level was 40 copies/g .
	manualset3
254009	3	423875	15	NULL	NULL	NULL	NULL	40 copies/g	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At admission , the EBV deoxyribonucleic acid ( DNA ) blood level was 40 copies/g .
	manualset3
254012	1	423876	15	NULL	NULL	NULL	NULL	tested intervals	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At all tested intervals after transplantation thymus grafts hardly differed from the recipient 's own thymus in immunohistology and lymphocyte yield .
	manualset3
254014	2	423876	15	NULL	NULL	NULL	NULL	transplantation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At all tested intervals after transplantation thymus grafts hardly differed from the recipient 's own thymus in immunohistology and lymphocyte yield .
	manualset3
254017	3	423876	15	NULL	NULL	NULL	NULL	thymus grafts	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At all tested intervals after transplantation thymus grafts hardly differed from the recipient 's own thymus in immunohistology and lymphocyte yield .
	manualset3
254018	4	423876	15	NULL	NULL	NULL	NULL	recipient 's own thymus	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At all tested intervals after transplantation thymus grafts hardly differed from the recipient 's own thymus in immunohistology and lymphocyte yield .
	manualset3
254024	5	423876	15	NULL	NULL	NULL	NULL	immunohistology yield	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At all tested intervals after transplantation thymus grafts hardly differed from the recipient 's own thymus in immunohistology and lymphocyte yield .
	manualset3
254029	6	423876	15	NULL	NULL	NULL	NULL	lymphocyte yield	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At all tested intervals after transplantation thymus grafts hardly differed from the recipient 's own thymus in immunohistology and lymphocyte yield .
	manualset3
254036	1	423877	15	NULL	NULL	NULL	NULL	autopsy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At autopsy , Blocq and Marinesco discovered an encapsulated tumor confined to the substantia nigra , contralateral to the affected side , and concluded that tremor in that particular case resulted from a midbrain lesion .
	manualset3
254039	2	423877	15	NULL	NULL	NULL	NULL	Blocq	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At autopsy , Blocq and Marinesco discovered an encapsulated tumor confined to the substantia nigra , contralateral to the affected side , and concluded that tremor in that particular case resulted from a midbrain lesion .
	manualset3
254040	3	423877	15	NULL	NULL	NULL	NULL	Marinesco 	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At autopsy , Blocq and Marinesco discovered an encapsulated tumor confined to the substantia nigra , contralateral to the affected side , and concluded that tremor in that particular case resulted from a midbrain lesion .
	manualset3
254041	4	423877	15	NULL	NULL	NULL	NULL	encapsulated tumor	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At autopsy , Blocq and Marinesco discovered an encapsulated tumor confined to the substantia nigra , contralateral to the affected side , and concluded that tremor in that particular case resulted from a midbrain lesion .
	manualset3
254042	5	423877	15	NULL	NULL	NULL	NULL	substantia nigra 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At autopsy , Blocq and Marinesco discovered an encapsulated tumor confined to the substantia nigra , contralateral to the affected side , and concluded that tremor in that particular case resulted from a midbrain lesion .
	manualset3
254044	6	423877	15	NULL	NULL	NULL	NULL	affected side	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At autopsy , Blocq and Marinesco discovered an encapsulated tumor confined to the substantia nigra , contralateral to the affected side , and concluded that tremor in that particular case resulted from a midbrain lesion .
	manualset3
254046	7	423877	15	NULL	NULL	NULL	NULL	tremor	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At autopsy , Blocq and Marinesco discovered an encapsulated tumor confined to the substantia nigra , contralateral to the affected side , and concluded that tremor in that particular case resulted from a midbrain lesion .
	manualset3
254049	8	423877	15	NULL	NULL	NULL	NULL	case 	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At autopsy , Blocq and Marinesco discovered an encapsulated tumor confined to the substantia nigra , contralateral to the affected side , and concluded that tremor in that particular case resulted from a midbrain lesion .
	manualset3
254051	9	423877	15	NULL	NULL	NULL	NULL	midbrain lesion	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At autopsy , Blocq and Marinesco discovered an encapsulated tumor confined to the substantia nigra , contralateral to the affected side , and concluded that tremor in that particular case resulted from a midbrain lesion .
	manualset3
254050	1	423878	15	NULL	NULL	NULL	NULL	baseline	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At baseline , height and weight were determined by self-report .
	manualset3
254052	2	423878	15	NULL	NULL	NULL	NULL	height	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At baseline , height and weight were determined by self-report .
	manualset3
254053	3	423878	15	NULL	NULL	NULL	NULL	weight	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At baseline , height and weight were determined by self-report .
	manualset3
254054	4	423878	15	NULL	NULL	NULL	NULL	self-report	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At baseline , height and weight were determined by self-report .
	manualset3
254055	1	423879	15	NULL	NULL	NULL	NULL	concentrations	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At concentrations exceeding critical micellization concentration complex formation is controlled by electrostatic association of protein with aggregates of the detergent 's molecules , stabilized , like micelles by hydrophobic forces .
	manualset3
254056	2	423879	15	NULL	NULL	NULL	NULL	critical micellization concentration	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At concentrations exceeding critical micellization concentration complex formation is controlled by electrostatic association of protein with aggregates of the detergent 's molecules , stabilized , like micelles by hydrophobic forces .
	manualset3
254057	3	423879	15	NULL	NULL	NULL	NULL	complex formation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At concentrations exceeding critical micellization concentration complex formation is controlled by electrostatic association of protein with aggregates of the detergent 's molecules , stabilized , like micelles by hydrophobic forces .
	manualset3
254060	4	423879	15	NULL	NULL	NULL	NULL	electrostatic association	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At concentrations exceeding critical micellization concentration complex formation is controlled by electrostatic association of protein with aggregates of the detergent 's molecules , stabilized , like micelles by hydrophobic forces .
	manualset3
254066	5	423879	15	NULL	NULL	NULL	NULL	protein	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At concentrations exceeding critical micellization concentration complex formation is controlled by electrostatic association of protein with aggregates of the detergent 's molecules , stabilized , like micelles by hydrophobic forces .
	manualset3
254069	6	423879	15	NULL	NULL	NULL	NULL	aggregates of the detergent 's molecules 	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At concentrations exceeding critical micellization concentration complex formation is controlled by electrostatic association of protein with aggregates of the detergent 's molecules , stabilized , like micelles by hydrophobic forces .
	manualset3
254071	7	423879	15	NULL	NULL	NULL	NULL	micelles	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At concentrations exceeding critical micellization concentration complex formation is controlled by electrostatic association of protein with aggregates of the detergent 's molecules , stabilized , like micelles by hydrophobic forces .
	manualset3
254072	8	423879	15	NULL	NULL	NULL	NULL	 hydrophobic forces 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At concentrations exceeding critical micellization concentration complex formation is controlled by electrostatic association of protein with aggregates of the detergent 's molecules , stabilized , like micelles by hydrophobic forces .
	manualset3
254080	1	423880	15	NULL	NULL	NULL	NULL	day 14 	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At day 14 , vasodilator treatment lowered hematocrit and increased PV ( determined by Evans blue dye dilution ) .
	manualset3
254081	2	423880	15	NULL	NULL	NULL	NULL	vasodilator treatment 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At day 14 , vasodilator treatment lowered hematocrit and increased PV ( determined by Evans blue dye dilution ) .
	manualset3
254082	3	423880	15	NULL	NULL	NULL	NULL	hematocrit	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At day 14 , vasodilator treatment lowered hematocrit and increased PV ( determined by Evans blue dye dilution ) .
	manualset3
254088	4	423880	15	NULL	NULL	NULL	NULL	PV	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At day 14 , vasodilator treatment lowered hematocrit and increased PV ( determined by Evans blue dye dilution ) .
	manualset3
254089	5	423880	15	NULL	NULL	NULL	NULL	Evans blue dye dilution 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At day 14 , vasodilator treatment lowered hematocrit and increased PV ( determined by Evans blue dye dilution ) .
	manualset3
254083	1	423881	15	NULL	NULL	NULL	NULL	Epicondylosis 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Epicondylosis and epithrocleosis with calcification : calcifying periarthritis of the elbow ) .
	manualset3
254084	2	423881	15	NULL	NULL	NULL	NULL	epithrocleosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Epicondylosis and epithrocleosis with calcification : calcifying periarthritis of the elbow ) .
	manualset3
254085	3	423881	15	NULL	NULL	NULL	NULL	calcification	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Epicondylosis and epithrocleosis with calcification : calcifying periarthritis of the elbow ) .
	manualset3
254086	4	423881	15	NULL	NULL	NULL	NULL	calcifying periarthritis 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Epicondylosis and epithrocleosis with calcification : calcifying periarthritis of the elbow ) .
	manualset3
254087	5	423881	15	NULL	NULL	NULL	NULL	elbow	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Epicondylosis and epithrocleosis with calcification : calcifying periarthritis of the elbow ) .
	manualset3
254094	1	423882	15	NULL	NULL	NULL	NULL	day 3	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At day 3 post drug administration , peritoneal macrophages were harvested by peritoneal lavage , and the phagocytic activity of the macrophages was determined by a chemiluminescence assay using opsonized zymosan particles .
	manualset3
254095	2	423882	15	NULL	NULL	NULL	NULL	post drug administration	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At day 3 post drug administration , peritoneal macrophages were harvested by peritoneal lavage , and the phagocytic activity of the macrophages was determined by a chemiluminescence assay using opsonized zymosan particles .
	manualset3
254096	3	423882	15	NULL	NULL	NULL	NULL	peritoneal macrophages	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At day 3 post drug administration , peritoneal macrophages were harvested by peritoneal lavage , and the phagocytic activity of the macrophages was determined by a chemiluminescence assay using opsonized zymosan particles .
	manualset3
254097	4	423882	15	NULL	NULL	NULL	NULL	peritoneal lavage	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At day 3 post drug administration , peritoneal macrophages were harvested by peritoneal lavage , and the phagocytic activity of the macrophages was determined by a chemiluminescence assay using opsonized zymosan particles .
	manualset3
254098	5	423882	15	NULL	NULL	NULL	NULL	phagocytic activity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At day 3 post drug administration , peritoneal macrophages were harvested by peritoneal lavage , and the phagocytic activity of the macrophages was determined by a chemiluminescence assay using opsonized zymosan particles .
	manualset3
254099	6	423882	15	NULL	NULL	NULL	NULL	macrophages	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At day 3 post drug administration , peritoneal macrophages were harvested by peritoneal lavage , and the phagocytic activity of the macrophages was determined by a chemiluminescence assay using opsonized zymosan particles .
	manualset3
254100	7	423882	15	NULL	NULL	NULL	NULL	chemiluminescence assay 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At day 3 post drug administration , peritoneal macrophages were harvested by peritoneal lavage , and the phagocytic activity of the macrophages was determined by a chemiluminescence assay using opsonized zymosan particles .
	manualset3
254101	8	423882	15	NULL	NULL	NULL	NULL	opsonized zymosan particles	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At day 3 post drug administration , peritoneal macrophages were harvested by peritoneal lavage , and the phagocytic activity of the macrophages was determined by a chemiluminescence assay using opsonized zymosan particles .
	manualset3
254102	1	423883	15	NULL	NULL	NULL	NULL	day 7	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At day 7 , the pH in L. 3074 , FS-3 , and L. 3074 + FS-3 ( 1 : 1 ) treatment decreased from 6.90 to 3.30 , 5.88 , and 3.48 , respectively .
	manualset3
254104	2	423883	15	NULL	NULL	NULL	NULL	pH	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At day 7 , the pH in L. 3074 , FS-3 , and L. 3074 + FS-3 ( 1 : 1 ) treatment decreased from 6.90 to 3.30 , 5.88 , and 3.48 , respectively .
	manualset3
254105	3	423883	15	NULL	NULL	NULL	NULL	L. 3074	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At day 7 , the pH in L. 3074 , FS-3 , and L. 3074 + FS-3 ( 1 : 1 ) treatment decreased from 6.90 to 3.30 , 5.88 , and 3.48 , respectively .
	manualset3
254106	4	423883	15	NULL	NULL	NULL	NULL	FS-3 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At day 7 , the pH in L. 3074 , FS-3 , and L. 3074 + FS-3 ( 1 : 1 ) treatment decreased from 6.90 to 3.30 , 5.88 , and 3.48 , respectively .
	manualset3
254107	5	423883	15	NULL	NULL	NULL	NULL	L. 3074 + FS-3 ( 1 : 1 ) 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At day 7 , the pH in L. 3074 , FS-3 , and L. 3074 + FS-3 ( 1 : 1 ) treatment decreased from 6.90 to 3.30 , 5.88 , and 3.48 , respectively .
	manualset3
254108	6	423883	15	NULL	NULL	NULL	NULL	treatment 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At day 7 , the pH in L. 3074 , FS-3 , and L. 3074 + FS-3 ( 1 : 1 ) treatment decreased from 6.90 to 3.30 , 5.88 , and 3.48 , respectively .
	manualset3
254586	7	423883	15	NULL	NULL	NULL	NULL	6.90 to 3.30	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At day 7 , the pH in L. 3074 , FS-3 , and L. 3074 + FS-3 ( 1 : 1 ) treatment decreased from 6.90 to 3.30 , 5.88 , and 3.48 , respectively .
	manualset3
254587	8	423883	15	NULL	NULL	NULL	NULL	6.90 to 5.88	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At day 7 , the pH in L. 3074 , FS-3 , and L. 3074 + FS-3 ( 1 : 1 ) treatment decreased from 6.90 to 3.30 , 5.88 , and 3.48 , respectively .
	manualset3
254589	9	423883	15	NULL	NULL	NULL	NULL	6.90 to 3.48	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At day 7 , the pH in L. 3074 , FS-3 , and L. 3074 + FS-3 ( 1 : 1 ) treatment decreased from 6.90 to 3.30 , 5.88 , and 3.48 , respectively .
	manualset3
254109	1	423884	15	NULL	NULL	NULL	NULL	steady states	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At different steady states the environment was controlled with respect to the concentrations of dissolved oxygen , carbon and nitrogen , the pH , and the temperature .
	manualset3
254110	2	423884	15	NULL	NULL	NULL	NULL	environment 	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At different steady states the environment was controlled with respect to the concentrations of dissolved oxygen , carbon and nitrogen , the pH , and the temperature .
	manualset3
254111	3	423884	15	NULL	NULL	NULL	NULL	concentrations	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At different steady states the environment was controlled with respect to the concentrations of dissolved oxygen , carbon and nitrogen , the pH , and the temperature .
	manualset3
254112	4	423884	15	NULL	NULL	NULL	NULL	oxygen 	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At different steady states the environment was controlled with respect to the concentrations of dissolved oxygen , carbon and nitrogen , the pH , and the temperature .
	manualset3
254113	5	423884	15	NULL	NULL	NULL	NULL	carbon	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At different steady states the environment was controlled with respect to the concentrations of dissolved oxygen , carbon and nitrogen , the pH , and the temperature .
	manualset3
254114	6	423884	15	NULL	NULL	NULL	NULL	nitrogen	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At different steady states the environment was controlled with respect to the concentrations of dissolved oxygen , carbon and nitrogen , the pH , and the temperature .
	manualset3
254115	7	423884	15	NULL	NULL	NULL	NULL	pH	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At different steady states the environment was controlled with respect to the concentrations of dissolved oxygen , carbon and nitrogen , the pH , and the temperature .
	manualset3
254116	8	423884	15	NULL	NULL	NULL	NULL	temperature	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At different steady states the environment was controlled with respect to the concentrations of dissolved oxygen , carbon and nitrogen , the pH , and the temperature .
	manualset3
254117	1	423885	15	NULL	NULL	NULL	NULL	preload	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At each preload , displacements in each of six degrees of freedom ( + / -0.3 mm AP and lateral translations , + / -0.2 mm axial translation , + / -1 degrees lateral bending and + / -0.8 degrees flexion/extension and torsional rotations ) were imposed .
	manualset3
254118	2	423885	15	NULL	NULL	NULL	NULL	displacements	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At each preload , displacements in each of six degrees of freedom ( + / -0.3 mm AP and lateral translations , + / -0.2 mm axial translation , + / -1 degrees lateral bending and + / -0.8 degrees flexion/extension and torsional rotations ) were imposed .
	manualset3
254119	3	423885	15	NULL	NULL	NULL	NULL	six degrees of freedom	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At each preload , displacements in each of six degrees of freedom ( + / -0.3 mm AP and lateral translations , + / -0.2 mm axial translation , + / -1 degrees lateral bending and + / -0.8 degrees flexion/extension and torsional rotations ) were imposed .
	manualset3
254120	4	423885	15	NULL	NULL	NULL	NULL	+ / -0.3 mm AP 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At each preload , displacements in each of six degrees of freedom ( + / -0.3 mm AP and lateral translations , + / -0.2 mm axial translation , + / -1 degrees lateral bending and + / -0.8 degrees flexion/extension and torsional rotations ) were imposed .
	manualset3
254121	5	423885	15	NULL	NULL	NULL	NULL	lateral translations 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At each preload , displacements in each of six degrees of freedom ( + / -0.3 mm AP and lateral translations , + / -0.2 mm axial translation , + / -1 degrees lateral bending and + / -0.8 degrees flexion/extension and torsional rotations ) were imposed .
	manualset3
254122	6	423885	15	NULL	NULL	NULL	NULL	+ / -0.2 mm axial translation	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At each preload , displacements in each of six degrees of freedom ( + / -0.3 mm AP and lateral translations , + / -0.2 mm axial translation , + / -1 degrees lateral bending and + / -0.8 degrees flexion/extension and torsional rotations ) were imposed .
	manualset3
254123	7	423885	15	NULL	NULL	NULL	NULL	+ / -1 degrees lateral bending	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At each preload , displacements in each of six degrees of freedom ( + / -0.3 mm AP and lateral translations , + / -0.2 mm axial translation , + / -1 degrees lateral bending and + / -0.8 degrees flexion/extension and torsional rotations ) were imposed .
	manualset3
254124	8	423885	15	NULL	NULL	NULL	NULL	+ / -0.8 degrees flexion/extension 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At each preload , displacements in each of six degrees of freedom ( + / -0.3 mm AP and lateral translations , + / -0.2 mm axial translation , + / -1 degrees lateral bending and + / -0.8 degrees flexion/extension and torsional rotations ) were imposed .
	manualset3
254125	9	423885	15	NULL	NULL	NULL	NULL	torsional rotations	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At each preload , displacements in each of six degrees of freedom ( + / -0.3 mm AP and lateral translations , + / -0.2 mm axial translation , + / -1 degrees lateral bending and + / -0.8 degrees flexion/extension and torsional rotations ) were imposed .
	manualset3
254126	1	423886	15	NULL	NULL	NULL	NULL	concentrations	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At extreme concentrations ( listed above ) , Cd accumulation was unaffected by the presence of Zn whereas Zn accumulation rates were reduced by 58 % .
	manualset3
254127	2	423886	15	NULL	NULL	NULL	NULL	Cd accumulation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At extreme concentrations ( listed above ) , Cd accumulation was unaffected by the presence of Zn whereas Zn accumulation rates were reduced by 58 % .
	manualset3
254128	3	423886	15	NULL	NULL	NULL	NULL	Zn	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At extreme concentrations ( listed above ) , Cd accumulation was unaffected by the presence of Zn whereas Zn accumulation rates were reduced by 58 % .
	manualset3
254129	4	423886	15	NULL	NULL	NULL	NULL	Zn accumulation rates	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At extreme concentrations ( listed above ) , Cd accumulation was unaffected by the presence of Zn whereas Zn accumulation rates were reduced by 58 % .
	manualset3
254130	5	423886	15	NULL	NULL	NULL	NULL	58 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At extreme concentrations ( listed above ) , Cd accumulation was unaffected by the presence of Zn whereas Zn accumulation rates were reduced by 58 % .
	manualset3
254131	1	423887	15	NULL	NULL	NULL	NULL	fertilization	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At fertilization , the highly condensed and transcriptionally inert chromatin of the spermatozoa becomes remodelled into the decondensed and transcriptionally competent chromatin of the male pronucleus .
	manualset3
254132	2	423887	15	NULL	NULL	NULL	NULL	chromatin	Chromosome												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At fertilization , the highly condensed and transcriptionally inert chromatin of the spermatozoa becomes remodelled into the decondensed and transcriptionally competent chromatin of the male pronucleus .
	manualset3
254133	3	423887	15	NULL	NULL	NULL	NULL	spermatozoa	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At fertilization , the highly condensed and transcriptionally inert chromatin of the spermatozoa becomes remodelled into the decondensed and transcriptionally competent chromatin of the male pronucleus .
	manualset3
254134	4	423887	15	NULL	NULL	NULL	NULL	chromatin	Chromosome												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At fertilization , the highly condensed and transcriptionally inert chromatin of the spermatozoa becomes remodelled into the decondensed and transcriptionally competent chromatin of the male pronucleus .
	manualset3
254135	5	423887	15	NULL	NULL	NULL	NULL	male pronucleus	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At fertilization , the highly condensed and transcriptionally inert chromatin of the spermatozoa becomes remodelled into the decondensed and transcriptionally competent chromatin of the male pronucleus .
	manualset3
254136	1	423888	15	NULL	NULL	NULL	NULL	follow up 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At follow up of the 51 patients with reciprocal changes in the ST segment 36 had become symptomatic , of whom 29 had undergone coronary artery bypass surgery .
	manualset3
254137	2	423888	15	NULL	NULL	NULL	NULL	51 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At follow up of the 51 patients with reciprocal changes in the ST segment 36 had become symptomatic , of whom 29 had undergone coronary artery bypass surgery .
	manualset3
254138	3	423888	15	NULL	NULL	NULL	NULL	reciprocal changes	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At follow up of the 51 patients with reciprocal changes in the ST segment 36 had become symptomatic , of whom 29 had undergone coronary artery bypass surgery .
	manualset3
254139	4	423888	15	NULL	NULL	NULL	NULL	ST segment	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At follow up of the 51 patients with reciprocal changes in the ST segment 36 had become symptomatic , of whom 29 had undergone coronary artery bypass surgery .
	manualset3
254140	6	423888	15	NULL	NULL	NULL	NULL	29	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At follow up of the 51 patients with reciprocal changes in the ST segment 36 had become symptomatic , of whom 29 had undergone coronary artery bypass surgery .
	manualset3
254141	7	423888	15	NULL	NULL	NULL	NULL	coronary artery bypass surgery	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At follow up of the 51 patients with reciprocal changes in the ST segment 36 had become symptomatic , of whom 29 had undergone coronary artery bypass surgery .
	manualset3
254142	5	423888	15	NULL	NULL	NULL	NULL	36	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At follow up of the 51 patients with reciprocal changes in the ST segment 36 had become symptomatic , of whom 29 had undergone coronary artery bypass surgery .
	manualset3
254143	1	423889	15	NULL	NULL	NULL	NULL	time-points	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At further time-points , AIx remained low , while AId progressively increased , to overshoot above preexercise at 45 min .
	manualset3
254145	2	423889	15	NULL	NULL	NULL	NULL	AIx	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At further time-points , AIx remained low , while AId progressively increased , to overshoot above preexercise at 45 min .
	manualset3
254147	3	423889	15	NULL	NULL	NULL	NULL	AId 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At further time-points , AIx remained low , while AId progressively increased , to overshoot above preexercise at 45 min .
	manualset3
254150	4	423889	15	NULL	NULL	NULL	NULL	preexercise	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At further time-points , AIx remained low , while AId progressively increased , to overshoot above preexercise at 45 min .
	manualset3
254151	5	423889	15	NULL	NULL	NULL	NULL	45 min	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At further time-points , AIx remained low , while AId progressively increased , to overshoot above preexercise at 45 min .
	manualset3
254154	1	423890	15	NULL	NULL	NULL	NULL	Epidemiology 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Epidemiology of depression ) .
	manualset3
254155	2	423890	15	NULL	NULL	NULL	NULL	depression	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Epidemiology of depression ) .
	manualset3
254158	1	423891	15	NULL	NULL	NULL	NULL	concentrations	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At high concentrations , the sulfhydryl reagent , thimerosal ( 200 microM ) , causes Ca2 + oscillations in eggs and produces similar oscillations in oocytes .
	manualset3
254160	2	423891	15	NULL	NULL	NULL	NULL	sulfhydryl reagent	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At high concentrations , the sulfhydryl reagent , thimerosal ( 200 microM ) , causes Ca2 + oscillations in eggs and produces similar oscillations in oocytes .
	manualset3
254162	3	423891	15	NULL	NULL	NULL	NULL	thimerosal	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At high concentrations , the sulfhydryl reagent , thimerosal ( 200 microM ) , causes Ca2 + oscillations in eggs and produces similar oscillations in oocytes .
	manualset3
254163	4	423891	15	NULL	NULL	NULL	NULL	200 microM	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At high concentrations , the sulfhydryl reagent , thimerosal ( 200 microM ) , causes Ca2 + oscillations in eggs and produces similar oscillations in oocytes .
	manualset3
254164	5	423891	15	NULL	NULL	NULL	NULL	Ca2 + oscillations 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At high concentrations , the sulfhydryl reagent , thimerosal ( 200 microM ) , causes Ca2 + oscillations in eggs and produces similar oscillations in oocytes .
	manualset3
254165	6	423891	15	NULL	NULL	NULL	NULL	eggs	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At high concentrations , the sulfhydryl reagent , thimerosal ( 200 microM ) , causes Ca2 + oscillations in eggs and produces similar oscillations in oocytes .
	manualset3
254166	7	423891	15	NULL	NULL	NULL	NULL	oscillations 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At high concentrations , the sulfhydryl reagent , thimerosal ( 200 microM ) , causes Ca2 + oscillations in eggs and produces similar oscillations in oocytes .
	manualset3
254168	8	423891	15	NULL	NULL	NULL	NULL	oocytes	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At high concentrations , the sulfhydryl reagent , thimerosal ( 200 microM ) , causes Ca2 + oscillations in eggs and produces similar oscillations in oocytes .
	manualset3
254173	1	423892	15	NULL	NULL	NULL	NULL	K +	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At high extravesicular K + , the addition of valinomycin reduced taurine uptake .
	manualset3
254175	2	423892	15	NULL	NULL	NULL	NULL	addition	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At high extravesicular K + , the addition of valinomycin reduced taurine uptake .
	manualset3
254177	3	423892	15	NULL	NULL	NULL	NULL	valinomycin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At high extravesicular K + , the addition of valinomycin reduced taurine uptake .
	manualset3
254180	4	423892	15	NULL	NULL	NULL	NULL	taurine uptake	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At high extravesicular K + , the addition of valinomycin reduced taurine uptake .
	manualset3
254185	1	423893	15	NULL	NULL	NULL	NULL	temperature	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At high temperature ( 26 -- 27 degrees ) with 0.001 and 0.005 % of boron in the media , P. caudatum was also seen to multiply normally .
	manualset3
254187	2	423893	15	NULL	NULL	NULL	NULL	26 -- 27 degrees	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At high temperature ( 26 -- 27 degrees ) with 0.001 and 0.005 % of boron in the media , P. caudatum was also seen to multiply normally .
	manualset3
254189	3	423893	15	NULL	NULL	NULL	NULL	0.001% of boron	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At high temperature ( 26 -- 27 degrees ) with 0.001 and 0.005 % of boron in the media , P. caudatum was also seen to multiply normally .
	manualset3
254190	4	423893	15	NULL	NULL	NULL	NULL	0.005 % of boron 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At high temperature ( 26 -- 27 degrees ) with 0.001 and 0.005 % of boron in the media , P. caudatum was also seen to multiply normally .
	manualset3
254195	5	423893	15	NULL	NULL	NULL	NULL	media	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At high temperature ( 26 -- 27 degrees ) with 0.001 and 0.005 % of boron in the media , P. caudatum was also seen to multiply normally .
	manualset3
254196	6	423893	15	NULL	NULL	NULL	NULL	P. caudatum	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At high temperature ( 26 -- 27 degrees ) with 0.001 and 0.005 % of boron in the media , P. caudatum was also seen to multiply normally .
	manualset3
254216	1	423894	15	NULL	NULL	NULL	NULL	speeds	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At higher speeds , muscle power appears to limit acceleration .
	manualset3
254217	2	423894	15	NULL	NULL	NULL	NULL	muscle power	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At higher speeds , muscle power appears to limit acceleration .
	manualset3
254218	3	423894	15	NULL	NULL	NULL	NULL	acceleration	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At higher speeds , muscle power appears to limit acceleration .
	manualset3
254219	1	423895	15	NULL	NULL	NULL	NULL	inclusion	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At inclusion , patients had low CD4 cell counts ( 27 cells/mm ( 3 ) ) and high plasma viral load ( 5.76 and 5.50 log/mL in IRIS and non-IRIS patients , respectively ) .
	manualset3
254220	2	423895	15	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At inclusion , patients had low CD4 cell counts ( 27 cells/mm ( 3 ) ) and high plasma viral load ( 5.76 and 5.50 log/mL in IRIS and non-IRIS patients , respectively ) .
	manualset3
254221	3	423895	15	NULL	NULL	NULL	NULL	CD4 cell counts	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At inclusion , patients had low CD4 cell counts ( 27 cells/mm ( 3 ) ) and high plasma viral load ( 5.76 and 5.50 log/mL in IRIS and non-IRIS patients , respectively ) .
	manualset3
254222	4	423895	15	NULL	NULL	NULL	NULL	27 cells/mm ( 3 )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At inclusion , patients had low CD4 cell counts ( 27 cells/mm ( 3 ) ) and high plasma viral load ( 5.76 and 5.50 log/mL in IRIS and non-IRIS patients , respectively ) .
	manualset3
254223	5	423895	15	NULL	NULL	NULL	NULL	plasma viral load	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At inclusion , patients had low CD4 cell counts ( 27 cells/mm ( 3 ) ) and high plasma viral load ( 5.76 and 5.50 log/mL in IRIS and non-IRIS patients , respectively ) .
	manualset3
254224	6	423895	15	NULL	NULL	NULL	NULL	5.76 log/mL	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At inclusion , patients had low CD4 cell counts ( 27 cells/mm ( 3 ) ) and high plasma viral load ( 5.76 and 5.50 log/mL in IRIS and non-IRIS patients , respectively ) .
	manualset3
254225	7	423895	15	NULL	NULL	NULL	NULL	5.50 log/mL	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At inclusion , patients had low CD4 cell counts ( 27 cells/mm ( 3 ) ) and high plasma viral load ( 5.76 and 5.50 log/mL in IRIS and non-IRIS patients , respectively ) .
	manualset3
254226	8	423895	15	NULL	NULL	NULL	NULL	IRIS patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At inclusion , patients had low CD4 cell counts ( 27 cells/mm ( 3 ) ) and high plasma viral load ( 5.76 and 5.50 log/mL in IRIS and non-IRIS patients , respectively ) .
	manualset3
254227	9	423895	15	NULL	NULL	NULL	NULL	non-IRIS patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At inclusion , patients had low CD4 cell counts ( 27 cells/mm ( 3 ) ) and high plasma viral load ( 5.76 and 5.50 log/mL in IRIS and non-IRIS patients , respectively ) .
	manualset3
254228	1	423896	15	NULL	NULL	NULL	NULL	5 ' end	Chromosome												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At its 5 ' end is an ORF encoding a protein of 227 kDa , distantly homologous to the multifunctional replicases of benyviruses and rubiviruses .
	manualset3
254229	2	423896	15	NULL	NULL	NULL	NULL	ORF	Chromosome												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At its 5 ' end is an ORF encoding a protein of 227 kDa , distantly homologous to the multifunctional replicases of benyviruses and rubiviruses .
	manualset3
254230	3	423896	15	NULL	NULL	NULL	NULL	protein 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At its 5 ' end is an ORF encoding a protein of 227 kDa , distantly homologous to the multifunctional replicases of benyviruses and rubiviruses .
	manualset3
254231	4	423896	15	NULL	NULL	NULL	NULL	227 kDa	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At its 5 ' end is an ORF encoding a protein of 227 kDa , distantly homologous to the multifunctional replicases of benyviruses and rubiviruses .
	manualset3
254232	5	423896	15	NULL	NULL	NULL	NULL	homologous 	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At its 5 ' end is an ORF encoding a protein of 227 kDa , distantly homologous to the multifunctional replicases of benyviruses and rubiviruses .
	manualset3
254233	6	423896	15	NULL	NULL	NULL	NULL	multifunctional replicases	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At its 5 ' end is an ORF encoding a protein of 227 kDa , distantly homologous to the multifunctional replicases of benyviruses and rubiviruses .
	manualset3
254234	7	423896	15	NULL	NULL	NULL	NULL	benyviruses 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At its 5 ' end is an ORF encoding a protein of 227 kDa , distantly homologous to the multifunctional replicases of benyviruses and rubiviruses .
	manualset3
254235	8	423896	15	NULL	NULL	NULL	NULL	rubiviruses	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At its 5 ' end is an ORF encoding a protein of 227 kDa , distantly homologous to the multifunctional replicases of benyviruses and rubiviruses .
	manualset3
254236	1	423897	15	NULL	NULL	NULL	NULL	current stage	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At its current stage the network model , built in BioTapestry , includes 22 genes encoding transcription factors , 4 genes encoding known signaling ligands , and 3 genes that are yet unknown but are predicted to perform specific roles .
	manualset3
254237	2	423897	15	NULL	NULL	NULL	NULL	network model	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At its current stage the network model , built in BioTapestry , includes 22 genes encoding transcription factors , 4 genes encoding known signaling ligands , and 3 genes that are yet unknown but are predicted to perform specific roles .
	manualset3
254238	3	423897	15	NULL	NULL	NULL	NULL	BioTapestry	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At its current stage the network model , built in BioTapestry , includes 22 genes encoding transcription factors , 4 genes encoding known signaling ligands , and 3 genes that are yet unknown but are predicted to perform specific roles .
	manualset3
254239	4	423897	15	NULL	NULL	NULL	NULL	22 genes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At its current stage the network model , built in BioTapestry , includes 22 genes encoding transcription factors , 4 genes encoding known signaling ligands , and 3 genes that are yet unknown but are predicted to perform specific roles .
	manualset3
254240	5	423897	15	NULL	NULL	NULL	NULL	transcription factors	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At its current stage the network model , built in BioTapestry , includes 22 genes encoding transcription factors , 4 genes encoding known signaling ligands , and 3 genes that are yet unknown but are predicted to perform specific roles .
	manualset3
254241	6	423897	15	NULL	NULL	NULL	NULL	4 genes 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At its current stage the network model , built in BioTapestry , includes 22 genes encoding transcription factors , 4 genes encoding known signaling ligands , and 3 genes that are yet unknown but are predicted to perform specific roles .
	manualset3
254242	7	423897	15	NULL	NULL	NULL	NULL	signaling ligands	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At its current stage the network model , built in BioTapestry , includes 22 genes encoding transcription factors , 4 genes encoding known signaling ligands , and 3 genes that are yet unknown but are predicted to perform specific roles .
	manualset3
254243	8	423897	15	NULL	NULL	NULL	NULL	3 genes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At its current stage the network model , built in BioTapestry , includes 22 genes encoding transcription factors , 4 genes encoding known signaling ligands , and 3 genes that are yet unknown but are predicted to perform specific roles .
	manualset3
254244	9	423897	15	NULL	NULL	NULL	NULL	roles	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At its current stage the network model , built in BioTapestry , includes 22 genes encoding transcription factors , 4 genes encoding known signaling ligands , and 3 genes that are yet unknown but are predicted to perform specific roles .
	manualset3
254246	1	423898	15	NULL	NULL	NULL	NULL	laparotomy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At laparotomy the tumor was found to be pendiculated and growing extramurally from the anterior wall of the stomach .
	manualset3
254247	2	423898	15	NULL	NULL	NULL	NULL	tumor	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At laparotomy the tumor was found to be pendiculated and growing extramurally from the anterior wall of the stomach .
	manualset3
254248	3	423898	15	NULL	NULL	NULL	NULL	anterior wall of the stomach	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At laparotomy the tumor was found to be pendiculated and growing extramurally from the anterior wall of the stomach .
	manualset3
254249	1	423899	15	NULL	NULL	NULL	NULL	effectiveness	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At last the effectiveness of ketanserin treatment appears moderately higher in lean than in obese hypertensives .
	manualset3
254250	2	423899	15	NULL	NULL	NULL	NULL	ketanserin treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At last the effectiveness of ketanserin treatment appears moderately higher in lean than in obese hypertensives .
	manualset3
254251	3	423899	15	NULL	NULL	NULL	NULL	lean hypertensives	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At last the effectiveness of ketanserin treatment appears moderately higher in lean than in obese hypertensives .
	manualset3
254252	4	423899	15	NULL	NULL	NULL	NULL	obese hypertensives	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At last the effectiveness of ketanserin treatment appears moderately higher in lean than in obese hypertensives .
	manualset3
254254	1	423900	15	NULL	NULL	NULL	NULL	late embryonic stage	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At late embryonic and early postnatal stages , Wnt / - catenin activity shifts to the cerebellar ventricular zone and to cells arising from this germinal center .
	manualset3
254255	2	423900	15	NULL	NULL	NULL	NULL	early postnatal stage	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At late embryonic and early postnatal stages , Wnt / - catenin activity shifts to the cerebellar ventricular zone and to cells arising from this germinal center .
	manualset3
254256	3	423900	15	NULL	NULL	NULL	NULL	Wnt / - catenin activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At late embryonic and early postnatal stages , Wnt / - catenin activity shifts to the cerebellar ventricular zone and to cells arising from this germinal center .
	manualset3
254257	4	423900	15	NULL	NULL	NULL	NULL	cerebellar ventricular zone	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At late embryonic and early postnatal stages , Wnt / - catenin activity shifts to the cerebellar ventricular zone and to cells arising from this germinal center .
	manualset3
254258	5	423900	15	NULL	NULL	NULL	NULL	cells 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At late embryonic and early postnatal stages , Wnt / - catenin activity shifts to the cerebellar ventricular zone and to cells arising from this germinal center .
	manualset3
254259	6	423900	15	NULL	NULL	NULL	NULL	germinal center	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At late embryonic and early postnatal stages , Wnt / - catenin activity shifts to the cerebellar ventricular zone and to cells arising from this germinal center .
	manualset3
254260	1	423901	15	NULL	NULL	NULL	NULL	Epidemiology	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Epidemiology of poliomyelitis in France ) .
	manualset3
254261	2	423901	15	NULL	NULL	NULL	NULL	poliomyelitis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Epidemiology of poliomyelitis in France ) .
	manualset3
254268	3	423901	15	NULL	NULL	NULL	NULL	France 	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Epidemiology of poliomyelitis in France ) .
	manualset3
254272	1	423902	15	NULL	NULL	NULL	NULL	follow-up 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At late follow-up ( ) 2 years after PTCA ) , 29 patients showed regional LV function improvement , 15 showed no improvement , 3 showed worsening and 3 patients had cardiac events ( 1 nonfatal myocardial infarction and 2 unstable angina pectoris ) .
	manualset3
254273	2	423902	15	NULL	NULL	NULL	NULL	2 years after PTCA	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At late follow-up ( ) 2 years after PTCA ) , 29 patients showed regional LV function improvement , 15 showed no improvement , 3 showed worsening and 3 patients had cardiac events ( 1 nonfatal myocardial infarction and 2 unstable angina pectoris ) .
	manualset3
254279	3	423902	15	NULL	NULL	NULL	NULL	29 patients 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At late follow-up ( ) 2 years after PTCA ) , 29 patients showed regional LV function improvement , 15 showed no improvement , 3 showed worsening and 3 patients had cardiac events ( 1 nonfatal myocardial infarction and 2 unstable angina pectoris ) .
	manualset3
254281	4	423902	15	NULL	NULL	NULL	NULL	regional LV function improvement	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At late follow-up ( ) 2 years after PTCA ) , 29 patients showed regional LV function improvement , 15 showed no improvement , 3 showed worsening and 3 patients had cardiac events ( 1 nonfatal myocardial infarction and 2 unstable angina pectoris ) .
	manualset3
254283	5	423902	15	NULL	NULL	NULL	NULL	15 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At late follow-up ( ) 2 years after PTCA ) , 29 patients showed regional LV function improvement , 15 showed no improvement , 3 showed worsening and 3 patients had cardiac events ( 1 nonfatal myocardial infarction and 2 unstable angina pectoris ) .
	manualset3
254285	6	423902	15	NULL	NULL	NULL	NULL	improvement	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At late follow-up ( ) 2 years after PTCA ) , 29 patients showed regional LV function improvement , 15 showed no improvement , 3 showed worsening and 3 patients had cardiac events ( 1 nonfatal myocardial infarction and 2 unstable angina pectoris ) .
	manualset3
254286	7	423902	15	NULL	NULL	NULL	NULL	3 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At late follow-up ( ) 2 years after PTCA ) , 29 patients showed regional LV function improvement , 15 showed no improvement , 3 showed worsening and 3 patients had cardiac events ( 1 nonfatal myocardial infarction and 2 unstable angina pectoris ) .
	manualset3
254289	8	423902	15	NULL	NULL	NULL	NULL	3 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At late follow-up ( ) 2 years after PTCA ) , 29 patients showed regional LV function improvement , 15 showed no improvement , 3 showed worsening and 3 patients had cardiac events ( 1 nonfatal myocardial infarction and 2 unstable angina pectoris ) .
	manualset3
254291	9	423902	15	NULL	NULL	NULL	NULL	cardiac events	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At late follow-up ( ) 2 years after PTCA ) , 29 patients showed regional LV function improvement , 15 showed no improvement , 3 showed worsening and 3 patients had cardiac events ( 1 nonfatal myocardial infarction and 2 unstable angina pectoris ) .
	manualset3
254292	10	423902	15	NULL	NULL	NULL	NULL	1 nonfatal myocardial infarction	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At late follow-up ( ) 2 years after PTCA ) , 29 patients showed regional LV function improvement , 15 showed no improvement , 3 showed worsening and 3 patients had cardiac events ( 1 nonfatal myocardial infarction and 2 unstable angina pectoris ) .
	manualset3
254293	11	423902	15	NULL	NULL	NULL	NULL	2 unstable angina pectoris	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At late follow-up ( ) 2 years after PTCA ) , 29 patients showed regional LV function improvement , 15 showed no improvement , 3 showed worsening and 3 patients had cardiac events ( 1 nonfatal myocardial infarction and 2 unstable angina pectoris ) .
	manualset3
254294	1	423903	15	NULL	NULL	NULL	NULL	later stages	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At later stages of SVDV cytopathology , cells showed a completely vacuolated cytoplasm containing vesicles of different sizes .
	manualset3
254295	2	423903	15	NULL	NULL	NULL	NULL	SVDV cytopathology	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At later stages of SVDV cytopathology , cells showed a completely vacuolated cytoplasm containing vesicles of different sizes .
	manualset3
254296	3	423903	15	NULL	NULL	NULL	NULL	cells 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At later stages of SVDV cytopathology , cells showed a completely vacuolated cytoplasm containing vesicles of different sizes .
	manualset3
254297	4	423903	15	NULL	NULL	NULL	NULL	cytoplasm 	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At later stages of SVDV cytopathology , cells showed a completely vacuolated cytoplasm containing vesicles of different sizes .
	manualset3
254304	5	423903	15	NULL	NULL	NULL	NULL	vesicles	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At later stages of SVDV cytopathology , cells showed a completely vacuolated cytoplasm containing vesicles of different sizes .
	manualset3
254305	6	423903	15	NULL	NULL	NULL	NULL	sizes	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At later stages of SVDV cytopathology , cells showed a completely vacuolated cytoplasm containing vesicles of different sizes .
	manualset3
254299	1	423904	15	NULL	NULL	NULL	NULL	 0.4 M guanidine-HCl	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At least 0.4 M guanidine-HCl is required to abolish the negative interference by proteins .
	manualset3
254300	2	423904	15	NULL	NULL	NULL	NULL	negative interference	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At least 0.4 M guanidine-HCl is required to abolish the negative interference by proteins .
	manualset3
254310	3	423904	15	NULL	NULL	NULL	NULL	proteins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At least 0.4 M guanidine-HCl is required to abolish the negative interference by proteins .
	manualset3
254313	1	423905	15	NULL	NULL	NULL	NULL	10.6 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At least 10.6 % of the red colobus diet and 8.8 % of the gorilla diet had estrogenic activity .
	manualset3
254314	2	423905	15	NULL	NULL	NULL	NULL	red colobus diet	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At least 10.6 % of the red colobus diet and 8.8 % of the gorilla diet had estrogenic activity .
	manualset3
254316	3	423905	15	NULL	NULL	NULL	NULL	8.8 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At least 10.6 % of the red colobus diet and 8.8 % of the gorilla diet had estrogenic activity .
	manualset3
254318	4	423905	15	NULL	NULL	NULL	NULL	gorilla diet 	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At least 10.6 % of the red colobus diet and 8.8 % of the gorilla diet had estrogenic activity .
	manualset3
254319	5	423905	15	NULL	NULL	NULL	NULL	estrogenic activity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At least 10.6 % of the red colobus diet and 8.8 % of the gorilla diet had estrogenic activity .
	manualset3
254323	1	423906	15	NULL	NULL	NULL	NULL	two systems of fibers 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At least two systems of fibers are associated with the basal bodies of all three genera .
	manualset3
254325	2	423906	15	NULL	NULL	NULL	NULL	basal bodies 	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At least two systems of fibers are associated with the basal bodies of all three genera .
	manualset3
254327	3	423906	15	NULL	NULL	NULL	NULL	three genera 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At least two systems of fibers are associated with the basal bodies of all three genera .
	manualset3
254330	1	423907	15	NULL	NULL	NULL	NULL	extent	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At least to some extent , the disappearance of unmyelinated ventral root axons from the juxtamedullary root fascicles was due to presence of intrafascicular axonal hairpin loops and to a shift of axons from ventral root fascicles to the pia mater .
	manualset3
254332	2	423907	15	NULL	NULL	NULL	NULL	disappearance of unmyelinated ventral root axons	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At least to some extent , the disappearance of unmyelinated ventral root axons from the juxtamedullary root fascicles was due to presence of intrafascicular axonal hairpin loops and to a shift of axons from ventral root fascicles to the pia mater .
	manualset3
254334	3	423907	15	NULL	NULL	NULL	NULL	juxtamedullary root fascicles	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At least to some extent , the disappearance of unmyelinated ventral root axons from the juxtamedullary root fascicles was due to presence of intrafascicular axonal hairpin loops and to a shift of axons from ventral root fascicles to the pia mater .
	manualset3
254335	4	423907	15	NULL	NULL	NULL	NULL	presence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At least to some extent , the disappearance of unmyelinated ventral root axons from the juxtamedullary root fascicles was due to presence of intrafascicular axonal hairpin loops and to a shift of axons from ventral root fascicles to the pia mater .
	manualset3
254339	5	423907	15	NULL	NULL	NULL	NULL	intrafascicular axonal hairpin loops 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At least to some extent , the disappearance of unmyelinated ventral root axons from the juxtamedullary root fascicles was due to presence of intrafascicular axonal hairpin loops and to a shift of axons from ventral root fascicles to the pia mater .
	manualset3
254344	6	423907	15	NULL	NULL	NULL	NULL	shift of axons	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At least to some extent , the disappearance of unmyelinated ventral root axons from the juxtamedullary root fascicles was due to presence of intrafascicular axonal hairpin loops and to a shift of axons from ventral root fascicles to the pia mater .
	manualset3
254345	7	423907	15	NULL	NULL	NULL	NULL	ventral root fascicles	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At least to some extent , the disappearance of unmyelinated ventral root axons from the juxtamedullary root fascicles was due to presence of intrafascicular axonal hairpin loops and to a shift of axons from ventral root fascicles to the pia mater .
	manualset3
254346	8	423907	15	NULL	NULL	NULL	NULL	pia mater	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At least to some extent , the disappearance of unmyelinated ventral root axons from the juxtamedullary root fascicles was due to presence of intrafascicular axonal hairpin loops and to a shift of axons from ventral root fascicles to the pia mater .
	manualset3
254364	1	423908	15	NULL	NULL	NULL	NULL	copy numbers	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At low copy numbers of the integrated vector , the transduced human lymphocytes exhibited high surface expression of the introduced tumor-specific TCR and reduced expression of endogenous TCRs .
	manualset3
254368	2	423908	15	NULL	NULL	NULL	NULL	integrated vector	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At low copy numbers of the integrated vector , the transduced human lymphocytes exhibited high surface expression of the introduced tumor-specific TCR and reduced expression of endogenous TCRs .
	manualset3
254410	3	423908	15	NULL	NULL	NULL	NULL	human lymphocytes	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At low copy numbers of the integrated vector , the transduced human lymphocytes exhibited high surface expression of the introduced tumor-specific TCR and reduced expression of endogenous TCRs .
	manualset3
254412	4	423908	15	NULL	NULL	NULL	NULL	high surface expression 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At low copy numbers of the integrated vector , the transduced human lymphocytes exhibited high surface expression of the introduced tumor-specific TCR and reduced expression of endogenous TCRs .
	manualset3
254416	5	423908	15	NULL	NULL	NULL	NULL	tumor-specific TCR 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At low copy numbers of the integrated vector , the transduced human lymphocytes exhibited high surface expression of the introduced tumor-specific TCR and reduced expression of endogenous TCRs .
	manualset3
254417	6	423908	15	NULL	NULL	NULL	NULL	reduced expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At low copy numbers of the integrated vector , the transduced human lymphocytes exhibited high surface expression of the introduced tumor-specific TCR and reduced expression of endogenous TCRs .
	manualset3
254427	7	423908	15	NULL	NULL	NULL	NULL	endogenous TCRs	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At low copy numbers of the integrated vector , the transduced human lymphocytes exhibited high surface expression of the introduced tumor-specific TCR and reduced expression of endogenous TCRs .
	manualset3
254430	1	423909	15	NULL	NULL	NULL	NULL	Epidemiology 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Epidemiology of postvaccinal encephalitis ) .
	manualset3
254433	2	423909	15	NULL	NULL	NULL	NULL	postvaccinal encephalitis 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Epidemiology of postvaccinal encephalitis ) .
	manualset3
254439	1	423910	15	NULL	NULL	NULL	NULL	solute concentrations	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At low solute concentrations , sorption of phenanthrene and naphthalene by biopolymer chars was dominated by the micropore-filling mechanism ; with an increase in the solute concentration , sorption of these two compounds by biopolymer chars shifted to a surface-sorption-dominant process .
	manualset3
254442	2	423910	15	NULL	NULL	NULL	NULL	sorption of phenanthrene	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At low solute concentrations , sorption of phenanthrene and naphthalene by biopolymer chars was dominated by the micropore-filling mechanism ; with an increase in the solute concentration , sorption of these two compounds by biopolymer chars shifted to a surface-sorption-dominant process .
	manualset3
254446	3	423910	15	NULL	NULL	NULL	NULL	sorption of naphthalene	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At low solute concentrations , sorption of phenanthrene and naphthalene by biopolymer chars was dominated by the micropore-filling mechanism ; with an increase in the solute concentration , sorption of these two compounds by biopolymer chars shifted to a surface-sorption-dominant process .
	manualset3
254450	4	423910	15	NULL	NULL	NULL	NULL	biopolymer chars	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At low solute concentrations , sorption of phenanthrene and naphthalene by biopolymer chars was dominated by the micropore-filling mechanism ; with an increase in the solute concentration , sorption of these two compounds by biopolymer chars shifted to a surface-sorption-dominant process .
	manualset3
254453	5	423910	15	NULL	NULL	NULL	NULL	micropore-filling mechanism 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At low solute concentrations , sorption of phenanthrene and naphthalene by biopolymer chars was dominated by the micropore-filling mechanism ; with an increase in the solute concentration , sorption of these two compounds by biopolymer chars shifted to a surface-sorption-dominant process .
	manualset3
254454	6	423910	15	NULL	NULL	NULL	NULL	increase	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At low solute concentrations , sorption of phenanthrene and naphthalene by biopolymer chars was dominated by the micropore-filling mechanism ; with an increase in the solute concentration , sorption of these two compounds by biopolymer chars shifted to a surface-sorption-dominant process .
	manualset3
254455	7	423910	15	NULL	NULL	NULL	NULL	solute concentration	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At low solute concentrations , sorption of phenanthrene and naphthalene by biopolymer chars was dominated by the micropore-filling mechanism ; with an increase in the solute concentration , sorption of these two compounds by biopolymer chars shifted to a surface-sorption-dominant process .
	manualset3
254456	8	423910	15	NULL	NULL	NULL	NULL	sorption 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At low solute concentrations , sorption of phenanthrene and naphthalene by biopolymer chars was dominated by the micropore-filling mechanism ; with an increase in the solute concentration , sorption of these two compounds by biopolymer chars shifted to a surface-sorption-dominant process .
	manualset3
254458	9	423910	15	NULL	NULL	NULL	NULL	two compounds	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At low solute concentrations , sorption of phenanthrene and naphthalene by biopolymer chars was dominated by the micropore-filling mechanism ; with an increase in the solute concentration , sorption of these two compounds by biopolymer chars shifted to a surface-sorption-dominant process .
	manualset3
254476	10	423910	15	NULL	NULL	NULL	NULL	biopolymer chars	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At low solute concentrations , sorption of phenanthrene and naphthalene by biopolymer chars was dominated by the micropore-filling mechanism ; with an increase in the solute concentration , sorption of these two compounds by biopolymer chars shifted to a surface-sorption-dominant process .
	manualset3
254483	11	423910	15	NULL	NULL	NULL	NULL	surface-sorption-dominant process 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At low solute concentrations , sorption of phenanthrene and naphthalene by biopolymer chars was dominated by the micropore-filling mechanism ; with an increase in the solute concentration , sorption of these two compounds by biopolymer chars shifted to a surface-sorption-dominant process .
	manualset3
254444	1	423911	15	NULL	NULL	NULL	NULL	ankle extensor contraction levels 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At matched ankle extensor contraction levels , stretch responses were compared before and after reversible block of the common peroneal nerve and during an attempted , voluntary , fictive dorsiflexion after common peroneal nerve block .
	manualset3
254457	2	423911	15	NULL	NULL	NULL	NULL	stretch responses	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At matched ankle extensor contraction levels , stretch responses were compared before and after reversible block of the common peroneal nerve and during an attempted , voluntary , fictive dorsiflexion after common peroneal nerve block .
	manualset3
254463	3	423911	15	NULL	NULL	NULL	NULL	reversible block of the common peroneal nerve	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At matched ankle extensor contraction levels , stretch responses were compared before and after reversible block of the common peroneal nerve and during an attempted , voluntary , fictive dorsiflexion after common peroneal nerve block .
	manualset3
254467	4	423911	15	NULL	NULL	NULL	NULL	fictive dorsiflexion 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At matched ankle extensor contraction levels , stretch responses were compared before and after reversible block of the common peroneal nerve and during an attempted , voluntary , fictive dorsiflexion after common peroneal nerve block .
	manualset3
254469	5	423911	15	NULL	NULL	NULL	NULL	peroneal nerve block	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At matched ankle extensor contraction levels , stretch responses were compared before and after reversible block of the common peroneal nerve and during an attempted , voluntary , fictive dorsiflexion after common peroneal nerve block .
	manualset3
254488	1	423912	15	NULL	NULL	NULL	NULL	multivariate analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At multivariate analysis the factors affecting renal prognosis were haematuria at presentation ( p & lt ; 0.05 , risk factor 3.52 ) , urinary protein/creatinine ratio ( p & lt ; 0.05 , risk factor 1.06 per 1 unit ) and low hemoglobin values ( p & lt ; 0.05 , risk factor 1.43 for each 1 g/dl decrement ) .
	manualset3
254490	2	423912	15	NULL	NULL	NULL	NULL	factors	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At multivariate analysis the factors affecting renal prognosis were haematuria at presentation ( p & lt ; 0.05 , risk factor 3.52 ) , urinary protein/creatinine ratio ( p & lt ; 0.05 , risk factor 1.06 per 1 unit ) and low hemoglobin values ( p & lt ; 0.05 , risk factor 1.43 for each 1 g/dl decrement ) .
	manualset3
254492	3	423912	15	NULL	NULL	NULL	NULL	renal prognosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At multivariate analysis the factors affecting renal prognosis were haematuria at presentation ( p & lt ; 0.05 , risk factor 3.52 ) , urinary protein/creatinine ratio ( p & lt ; 0.05 , risk factor 1.06 per 1 unit ) and low hemoglobin values ( p & lt ; 0.05 , risk factor 1.43 for each 1 g/dl decrement ) .
	manualset3
254496	4	423912	15	NULL	NULL	NULL	NULL	haematuria at presentation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At multivariate analysis the factors affecting renal prognosis were haematuria at presentation ( p & lt ; 0.05 , risk factor 3.52 ) , urinary protein/creatinine ratio ( p & lt ; 0.05 , risk factor 1.06 per 1 unit ) and low hemoglobin values ( p & lt ; 0.05 , risk factor 1.43 for each 1 g/dl decrement ) .
	manualset3
254506	5	423912	15	NULL	NULL	NULL	NULL	 p & lt ; 0.05	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At multivariate analysis the factors affecting renal prognosis were haematuria at presentation ( p & lt ; 0.05 , risk factor 3.52 ) , urinary protein/creatinine ratio ( p & lt ; 0.05 , risk factor 1.06 per 1 unit ) and low hemoglobin values ( p & lt ; 0.05 , risk factor 1.43 for each 1 g/dl decrement ) .
	manualset3
254507	6	423912	15	NULL	NULL	NULL	NULL	risk factor 3.52	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At multivariate analysis the factors affecting renal prognosis were haematuria at presentation ( p & lt ; 0.05 , risk factor 3.52 ) , urinary protein/creatinine ratio ( p & lt ; 0.05 , risk factor 1.06 per 1 unit ) and low hemoglobin values ( p & lt ; 0.05 , risk factor 1.43 for each 1 g/dl decrement ) .
	manualset3
254508	7	423912	15	NULL	NULL	NULL	NULL	urinary protein/creatinine ratio	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At multivariate analysis the factors affecting renal prognosis were haematuria at presentation ( p & lt ; 0.05 , risk factor 3.52 ) , urinary protein/creatinine ratio ( p & lt ; 0.05 , risk factor 1.06 per 1 unit ) and low hemoglobin values ( p & lt ; 0.05 , risk factor 1.43 for each 1 g/dl decrement ) .
	manualset3
254509	8	423912	15	NULL	NULL	NULL	NULL	p & lt ; 0.05	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At multivariate analysis the factors affecting renal prognosis were haematuria at presentation ( p & lt ; 0.05 , risk factor 3.52 ) , urinary protein/creatinine ratio ( p & lt ; 0.05 , risk factor 1.06 per 1 unit ) and low hemoglobin values ( p & lt ; 0.05 , risk factor 1.43 for each 1 g/dl decrement ) .
	manualset3
254510	9	423912	15	NULL	NULL	NULL	NULL	risk factor 1.06 per 1 unit 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At multivariate analysis the factors affecting renal prognosis were haematuria at presentation ( p & lt ; 0.05 , risk factor 3.52 ) , urinary protein/creatinine ratio ( p & lt ; 0.05 , risk factor 1.06 per 1 unit ) and low hemoglobin values ( p & lt ; 0.05 , risk factor 1.43 for each 1 g/dl decrement ) .
	manualset3
254512	10	423912	15	NULL	NULL	NULL	NULL	hemoglobin values	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At multivariate analysis the factors affecting renal prognosis were haematuria at presentation ( p & lt ; 0.05 , risk factor 3.52 ) , urinary protein/creatinine ratio ( p & lt ; 0.05 , risk factor 1.06 per 1 unit ) and low hemoglobin values ( p & lt ; 0.05 , risk factor 1.43 for each 1 g/dl decrement ) .
	manualset3
254515	11	423912	15	NULL	NULL	NULL	NULL	 p & lt ; 0.05	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At multivariate analysis the factors affecting renal prognosis were haematuria at presentation ( p & lt ; 0.05 , risk factor 3.52 ) , urinary protein/creatinine ratio ( p & lt ; 0.05 , risk factor 1.06 per 1 unit ) and low hemoglobin values ( p & lt ; 0.05 , risk factor 1.43 for each 1 g/dl decrement ) .
	manualset3
254519	12	423912	15	NULL	NULL	NULL	NULL	risk factor 1.43	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At multivariate analysis the factors affecting renal prognosis were haematuria at presentation ( p & lt ; 0.05 , risk factor 3.52 ) , urinary protein/creatinine ratio ( p & lt ; 0.05 , risk factor 1.06 per 1 unit ) and low hemoglobin values ( p & lt ; 0.05 , risk factor 1.43 for each 1 g/dl decrement ) .
	manualset3
254521	13	423912	15	NULL	NULL	NULL	NULL	1 g/dl decrement	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At multivariate analysis the factors affecting renal prognosis were haematuria at presentation ( p & lt ; 0.05 , risk factor 3.52 ) , urinary protein/creatinine ratio ( p & lt ; 0.05 , risk factor 1.06 per 1 unit ) and low hemoglobin values ( p & lt ; 0.05 , risk factor 1.43 for each 1 g/dl decrement ) .
	manualset3
254523	1	423913	15	NULL	NULL	NULL	NULL	nanosize level	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At nanosize level , helper hydrophilic polymers were used to impart the desired surface , bulk and release properties to PLGA NPs prepared by a modified emulsion-solvent diffusion technique .
	manualset3
254524	3	423913	15	NULL	NULL	NULL	NULL	surface properties 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At nanosize level , helper hydrophilic polymers were used to impart the desired surface , bulk and release properties to PLGA NPs prepared by a modified emulsion-solvent diffusion technique .
	manualset3
254526	2	423913	15	NULL	NULL	NULL	NULL	helper hydrophilic polymers	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At nanosize level , helper hydrophilic polymers were used to impart the desired surface , bulk and release properties to PLGA NPs prepared by a modified emulsion-solvent diffusion technique .
	manualset3
254529	4	423913	15	NULL	NULL	NULL	NULL	bulk properties 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At nanosize level , helper hydrophilic polymers were used to impart the desired surface , bulk and release properties to PLGA NPs prepared by a modified emulsion-solvent diffusion technique .
	manualset3
254531	5	423913	15	NULL	NULL	NULL	NULL	release properties 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At nanosize level , helper hydrophilic polymers were used to impart the desired surface , bulk and release properties to PLGA NPs prepared by a modified emulsion-solvent diffusion technique .
	manualset3
254535	6	423913	15	NULL	NULL	NULL	NULL	PLGA NPs	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At nanosize level , helper hydrophilic polymers were used to impart the desired surface , bulk and release properties to PLGA NPs prepared by a modified emulsion-solvent diffusion technique .
	manualset3
254538	7	423913	15	NULL	NULL	NULL	NULL	modified emulsion-solvent diffusion technique	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At nanosize level , helper hydrophilic polymers were used to impart the desired surface , bulk and release properties to PLGA NPs prepared by a modified emulsion-solvent diffusion technique .
	manualset3
254544	1	423914	15	NULL	NULL	NULL	NULL	one week	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At one , three , and six weeks , plasma levels of pentoxifylline and major derivatives were consistently detectable .
	manualset3
254554	2	423914	15	NULL	NULL	NULL	NULL	three weeks	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At one , three , and six weeks , plasma levels of pentoxifylline and major derivatives were consistently detectable .
	manualset3
254556	3	423914	15	NULL	NULL	NULL	NULL	six weeks	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At one , three , and six weeks , plasma levels of pentoxifylline and major derivatives were consistently detectable .
	manualset3
254558	4	423914	15	NULL	NULL	NULL	NULL	plasma levels	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At one , three , and six weeks , plasma levels of pentoxifylline and major derivatives were consistently detectable .
	manualset3
254560	5	423914	15	NULL	NULL	NULL	NULL	pentoxifylline	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At one , three , and six weeks , plasma levels of pentoxifylline and major derivatives were consistently detectable .
	manualset3
254561	6	423914	15	NULL	NULL	NULL	NULL	major derivatives	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At one , three , and six weeks , plasma levels of pentoxifylline and major derivatives were consistently detectable .
	manualset3
254564	1	423915	15	NULL	NULL	NULL	NULL	institution	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At our institution a targeted fetal cardiac exam is now used to confirm and provide detailed assessment of the heart anatomy when a screening fetal exam is positive for heart disease .
	manualset3
254565	2	423915	15	NULL	NULL	NULL	NULL	targeted fetal cardiac exam	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At our institution a targeted fetal cardiac exam is now used to confirm and provide detailed assessment of the heart anatomy when a screening fetal exam is positive for heart disease .
	manualset3
254607	3	423915	15	NULL	NULL	NULL	NULL	assessment of the heart anatomy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At our institution a targeted fetal cardiac exam is now used to confirm and provide detailed assessment of the heart anatomy when a screening fetal exam is positive for heart disease .
	manualset3
254610	4	423915	15	NULL	NULL	NULL	NULL	screening fetal exam	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At our institution a targeted fetal cardiac exam is now used to confirm and provide detailed assessment of the heart anatomy when a screening fetal exam is positive for heart disease .
	manualset3
254611	5	423915	15	NULL	NULL	NULL	NULL	heart disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At our institution a targeted fetal cardiac exam is now used to confirm and provide detailed assessment of the heart anatomy when a screening fetal exam is positive for heart disease .
	manualset3
254612	1	423916	15	NULL	NULL	NULL	NULL	Epidemiology	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Epidemiology of sarcoidosis in Japan ( author 's transl ) ) .
	manualset3
254613	2	423916	15	NULL	NULL	NULL	NULL	sarcoidosis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Epidemiology of sarcoidosis in Japan ( author 's transl ) ) .
	manualset3
254614	3	423916	15	NULL	NULL	NULL	NULL	Japan	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Epidemiology of sarcoidosis in Japan ( author 's transl ) ) .
	manualset3
254615	4	423916	15	NULL	NULL	NULL	NULL	author 's transl	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Epidemiology of sarcoidosis in Japan ( author 's transl ) ) .
	manualset3
254616	1	423917	15	NULL	NULL	NULL	NULL	positions five	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At positions five and six , a lysine residue and a valine residue , respectively , have replaced arginine and leucine residues found in the mouse sequence .
	manualset3
254617	2	423917	15	NULL	NULL	NULL	NULL	positions six	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At positions five and six , a lysine residue and a valine residue , respectively , have replaced arginine and leucine residues found in the mouse sequence .
	manualset3
254618	3	423917	15	NULL	NULL	NULL	NULL	lysine residue 	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At positions five and six , a lysine residue and a valine residue , respectively , have replaced arginine and leucine residues found in the mouse sequence .
	manualset3
254619	4	423917	15	NULL	NULL	NULL	NULL	valine residue	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At positions five and six , a lysine residue and a valine residue , respectively , have replaced arginine and leucine residues found in the mouse sequence .
	manualset3
254620	5	423917	15	NULL	NULL	NULL	NULL	arginine residue	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At positions five and six , a lysine residue and a valine residue , respectively , have replaced arginine and leucine residues found in the mouse sequence .
	manualset3
254622	6	423917	15	NULL	NULL	NULL	NULL	leucine residue	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At positions five and six , a lysine residue and a valine residue , respectively , have replaced arginine and leucine residues found in the mouse sequence .
	manualset3
254625	7	423917	15	NULL	NULL	NULL	NULL	mouse 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At positions five and six , a lysine residue and a valine residue , respectively , have replaced arginine and leucine residues found in the mouse sequence .
	manualset3
254626	8	423917	15	NULL	NULL	NULL	NULL	sequence 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At positions five and six , a lysine residue and a valine residue , respectively , have replaced arginine and leucine residues found in the mouse sequence .
	manualset3
254621	1	423918	15	NULL	NULL	NULL	NULL	present	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At present , little is known about how these interactions contribute to the mismatch repair mechanism .
	manualset3
254623	2	423918	15	NULL	NULL	NULL	NULL	interactions 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At present , little is known about how these interactions contribute to the mismatch repair mechanism .
	manualset3
254624	3	423918	15	NULL	NULL	NULL	NULL	mismatch repair mechanism	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At present , little is known about how these interactions contribute to the mismatch repair mechanism .
	manualset3
254635	1	423919	15	NULL	NULL	NULL	NULL	present	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At present , the functional significance of orexin afferents to MSDB is unclear , and the present study investigated a possible involvement of orexin innervation of the MSDB in spatial memory .
	manualset3
254639	2	423919	15	NULL	NULL	NULL	NULL	functional significance of orexin afferents	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At present , the functional significance of orexin afferents to MSDB is unclear , and the present study investigated a possible involvement of orexin innervation of the MSDB in spatial memory .
	manualset3
254641	3	423919	15	NULL	NULL	NULL	NULL	MSDB	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At present , the functional significance of orexin afferents to MSDB is unclear , and the present study investigated a possible involvement of orexin innervation of the MSDB in spatial memory .
	manualset3
254642	4	423919	15	NULL	NULL	NULL	NULL	present study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At present , the functional significance of orexin afferents to MSDB is unclear , and the present study investigated a possible involvement of orexin innervation of the MSDB in spatial memory .
	manualset3
254644	5	423919	15	NULL	NULL	NULL	NULL	involvement 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At present , the functional significance of orexin afferents to MSDB is unclear , and the present study investigated a possible involvement of orexin innervation of the MSDB in spatial memory .
	manualset3
254646	6	423919	15	NULL	NULL	NULL	NULL	orexin innervation of the MSDB	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At present , the functional significance of orexin afferents to MSDB is unclear , and the present study investigated a possible involvement of orexin innervation of the MSDB in spatial memory .
	manualset3
254648	7	423919	15	NULL	NULL	NULL	NULL	spatial memory	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At present , the functional significance of orexin afferents to MSDB is unclear , and the present study investigated a possible involvement of orexin innervation of the MSDB in spatial memory .
	manualset3
254653	1	423920	15	NULL	NULL	NULL	NULL	present	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At present , the titanium implant and resection using a template are more convincing due to the higher precision and practicability .
	manualset3
254659	2	423920	15	NULL	NULL	NULL	NULL	titanium implant	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At present , the titanium implant and resection using a template are more convincing due to the higher precision and practicability .
	manualset3
254661	3	423920	15	NULL	NULL	NULL	NULL	resection using a template 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At present , the titanium implant and resection using a template are more convincing due to the higher precision and practicability .
	manualset3
254665	4	423920	15	NULL	NULL	NULL	NULL	precision	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At present , the titanium implant and resection using a template are more convincing due to the higher precision and practicability .
	manualset3
254667	5	423920	15	NULL	NULL	NULL	NULL	practicability	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At present , the titanium implant and resection using a template are more convincing due to the higher precision and practicability .
	manualset3
255122	1	423921	15	NULL	NULL	NULL	NULL	saturating concentrations	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At saturating concentrations , about 8.2 micromol of protein was bound per g of bacterial microcrystalline cellulose , while Avicel , colloidal Avicel , and phosphoric acid-swollen cellulose bound 0.28 , 0.38 , and 0.55 micromol of miniCipC1 per g , respectively .
	manualset3
255123	2	423921	15	NULL	NULL	NULL	NULL	8.2 micromol 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At saturating concentrations , about 8.2 micromol of protein was bound per g of bacterial microcrystalline cellulose , while Avicel , colloidal Avicel , and phosphoric acid-swollen cellulose bound 0.28 , 0.38 , and 0.55 micromol of miniCipC1 per g , respectively .
	manualset3
255124	3	423921	15	NULL	NULL	NULL	NULL	protein 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At saturating concentrations , about 8.2 micromol of protein was bound per g of bacterial microcrystalline cellulose , while Avicel , colloidal Avicel , and phosphoric acid-swollen cellulose bound 0.28 , 0.38 , and 0.55 micromol of miniCipC1 per g , respectively .
	manualset3
255125	4	423921	15	NULL	NULL	NULL	NULL	g 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At saturating concentrations , about 8.2 micromol of protein was bound per g of bacterial microcrystalline cellulose , while Avicel , colloidal Avicel , and phosphoric acid-swollen cellulose bound 0.28 , 0.38 , and 0.55 micromol of miniCipC1 per g , respectively .
	manualset3
255126	5	423921	15	NULL	NULL	NULL	NULL	bacterial microcrystalline cellulose	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At saturating concentrations , about 8.2 micromol of protein was bound per g of bacterial microcrystalline cellulose , while Avicel , colloidal Avicel , and phosphoric acid-swollen cellulose bound 0.28 , 0.38 , and 0.55 micromol of miniCipC1 per g , respectively .
	manualset3
255127	6	423921	15	NULL	NULL	NULL	NULL	Avicel	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At saturating concentrations , about 8.2 micromol of protein was bound per g of bacterial microcrystalline cellulose , while Avicel , colloidal Avicel , and phosphoric acid-swollen cellulose bound 0.28 , 0.38 , and 0.55 micromol of miniCipC1 per g , respectively .
	manualset3
255128	7	423921	15	NULL	NULL	NULL	NULL	colloidal Avicel	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At saturating concentrations , about 8.2 micromol of protein was bound per g of bacterial microcrystalline cellulose , while Avicel , colloidal Avicel , and phosphoric acid-swollen cellulose bound 0.28 , 0.38 , and 0.55 micromol of miniCipC1 per g , respectively .
	manualset3
255129	8	423921	15	NULL	NULL	NULL	NULL	phosphoric acid-swollen cellulose	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At saturating concentrations , about 8.2 micromol of protein was bound per g of bacterial microcrystalline cellulose , while Avicel , colloidal Avicel , and phosphoric acid-swollen cellulose bound 0.28 , 0.38 , and 0.55 micromol of miniCipC1 per g , respectively .
	manualset3
255131	9	423921	15	NULL	NULL	NULL	NULL	0.28 micromol 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At saturating concentrations , about 8.2 micromol of protein was bound per g of bacterial microcrystalline cellulose , while Avicel , colloidal Avicel , and phosphoric acid-swollen cellulose bound 0.28 , 0.38 , and 0.55 micromol of miniCipC1 per g , respectively .
	manualset3
255132	10	423921	15	NULL	NULL	NULL	NULL	0.38 micromol 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At saturating concentrations , about 8.2 micromol of protein was bound per g of bacterial microcrystalline cellulose , while Avicel , colloidal Avicel , and phosphoric acid-swollen cellulose bound 0.28 , 0.38 , and 0.55 micromol of miniCipC1 per g , respectively .
	manualset3
255133	11	423921	15	NULL	NULL	NULL	NULL	0.55 micromol 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At saturating concentrations , about 8.2 micromol of protein was bound per g of bacterial microcrystalline cellulose , while Avicel , colloidal Avicel , and phosphoric acid-swollen cellulose bound 0.28 , 0.38 , and 0.55 micromol of miniCipC1 per g , respectively .
	manualset3
255134	12	423921	15	NULL	NULL	NULL	NULL	miniCipC1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At saturating concentrations , about 8.2 micromol of protein was bound per g of bacterial microcrystalline cellulose , while Avicel , colloidal Avicel , and phosphoric acid-swollen cellulose bound 0.28 , 0.38 , and 0.55 micromol of miniCipC1 per g , respectively .
	manualset3
255135	13	423921	15	NULL	NULL	NULL	NULL	g 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At saturating concentrations , about 8.2 micromol of protein was bound per g of bacterial microcrystalline cellulose , while Avicel , colloidal Avicel , and phosphoric acid-swollen cellulose bound 0.28 , 0.38 , and 0.55 micromol of miniCipC1 per g , respectively .
	manualset3
255136	1	423922	15	NULL	NULL	NULL	NULL	sites of inflammation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At sites of inflammation , endothelial cells play a major role in defining the types of leukocytes that are recruited to a specific area .
	manualset3
255137	2	423922	15	NULL	NULL	NULL	NULL	endothelial cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At sites of inflammation , endothelial cells play a major role in defining the types of leukocytes that are recruited to a specific area .
	manualset3
255138	3	423922	15	NULL	NULL	NULL	NULL	role	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At sites of inflammation , endothelial cells play a major role in defining the types of leukocytes that are recruited to a specific area .
	manualset3
255139	4	423922	15	NULL	NULL	NULL	NULL	types of leukocytes	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At sites of inflammation , endothelial cells play a major role in defining the types of leukocytes that are recruited to a specific area .
	manualset3
255140	5	423922	15	NULL	NULL	NULL	NULL	area	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At sites of inflammation , endothelial cells play a major role in defining the types of leukocytes that are recruited to a specific area .
	manualset3
255141	1	423923	15	NULL	NULL	NULL	NULL	six months	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At six months , tacrolimus was continued at 1-2 mg/day in 27 of 32 patients , but was discontinued in five cases who showed no or inadequate response .
	manualset3
255142	2	423923	15	NULL	NULL	NULL	NULL	tacrolimus	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At six months , tacrolimus was continued at 1-2 mg/day in 27 of 32 patients , but was discontinued in five cases who showed no or inadequate response .
	manualset3
255143	3	423923	15	NULL	NULL	NULL	NULL	1-2 mg/day	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At six months , tacrolimus was continued at 1-2 mg/day in 27 of 32 patients , but was discontinued in five cases who showed no or inadequate response .
	manualset3
255144	4	423923	15	NULL	NULL	NULL	NULL	27 of 32 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At six months , tacrolimus was continued at 1-2 mg/day in 27 of 32 patients , but was discontinued in five cases who showed no or inadequate response .
	manualset3
255145	5	423923	15	NULL	NULL	NULL	NULL	five cases	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At six months , tacrolimus was continued at 1-2 mg/day in 27 of 32 patients , but was discontinued in five cases who showed no or inadequate response .
	manualset3
255146	6	423923	15	NULL	NULL	NULL	NULL	inadequate response	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At six months , tacrolimus was continued at 1-2 mg/day in 27 of 32 patients , but was discontinued in five cases who showed no or inadequate response .
	manualset3
255147	1	423924	15	NULL	NULL	NULL	NULL	surgery	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At surgery , upon incision of the paravertebral muscle fascia , viscous pale fluid was encountered emanating from a foramen in the thoracic lamina .
	manualset3
255148	2	423924	15	NULL	NULL	NULL	NULL	incision of the paravertebral muscle fascia	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At surgery , upon incision of the paravertebral muscle fascia , viscous pale fluid was encountered emanating from a foramen in the thoracic lamina .
	manualset3
255150	3	423924	15	NULL	NULL	NULL	NULL	viscous pale fluid	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At surgery , upon incision of the paravertebral muscle fascia , viscous pale fluid was encountered emanating from a foramen in the thoracic lamina .
	manualset3
255151	4	423924	15	NULL	NULL	NULL	NULL	foramen	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At surgery , upon incision of the paravertebral muscle fascia , viscous pale fluid was encountered emanating from a foramen in the thoracic lamina .
	manualset3
255152	5	423924	15	NULL	NULL	NULL	NULL	thoracic lamina 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At surgery , upon incision of the paravertebral muscle fascia , viscous pale fluid was encountered emanating from a foramen in the thoracic lamina .
	manualset3
255153	1	423925	15	NULL	NULL	NULL	NULL	Epidemiology	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Epidemiology of transmissible gastroenteritis ( TGE ) of swine ) .
	manualset3
255155	2	423925	15	NULL	NULL	NULL	NULL	transmissible gastroenteritis ( TGE ) 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Epidemiology of transmissible gastroenteritis ( TGE ) of swine ) .
	manualset3
255156	3	423925	15	NULL	NULL	NULL	NULL	swine	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Epidemiology of transmissible gastroenteritis ( TGE ) of swine ) .
	manualset3
255157	1	423926	15	NULL	NULL	NULL	NULL	tail frequencies	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At tail frequencies , ANF phase changed with sound level ( often by 90 degrees-180 degrees ) and the deltaphi from a fiber was positively correlated with the slope of its phase-versus-sound-level function at the same frequency , as if deltaphi were caused by a 2-4 dB increase in sound level .
	manualset3
255158	2	423926	15	NULL	NULL	NULL	NULL	ANF phase	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At tail frequencies , ANF phase changed with sound level ( often by 90 degrees-180 degrees ) and the deltaphi from a fiber was positively correlated with the slope of its phase-versus-sound-level function at the same frequency , as if deltaphi were caused by a 2-4 dB increase in sound level .
	manualset3
255159	3	423926	15	NULL	NULL	NULL	NULL	sound level 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At tail frequencies , ANF phase changed with sound level ( often by 90 degrees-180 degrees ) and the deltaphi from a fiber was positively correlated with the slope of its phase-versus-sound-level function at the same frequency , as if deltaphi were caused by a 2-4 dB increase in sound level .
	manualset3
255160	4	423926	15	NULL	NULL	NULL	NULL	90 degrees-180 degrees	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At tail frequencies , ANF phase changed with sound level ( often by 90 degrees-180 degrees ) and the deltaphi from a fiber was positively correlated with the slope of its phase-versus-sound-level function at the same frequency , as if deltaphi were caused by a 2-4 dB increase in sound level .
	manualset3
255162	5	423926	15	NULL	NULL	NULL	NULL	deltaphi	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At tail frequencies , ANF phase changed with sound level ( often by 90 degrees-180 degrees ) and the deltaphi from a fiber was positively correlated with the slope of its phase-versus-sound-level function at the same frequency , as if deltaphi were caused by a 2-4 dB increase in sound level .
	manualset3
255164	6	423926	15	NULL	NULL	NULL	NULL	 fiber	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At tail frequencies , ANF phase changed with sound level ( often by 90 degrees-180 degrees ) and the deltaphi from a fiber was positively correlated with the slope of its phase-versus-sound-level function at the same frequency , as if deltaphi were caused by a 2-4 dB increase in sound level .
	manualset3
255165	7	423926	15	NULL	NULL	NULL	NULL	slope of its phase-versus-sound-level function 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At tail frequencies , ANF phase changed with sound level ( often by 90 degrees-180 degrees ) and the deltaphi from a fiber was positively correlated with the slope of its phase-versus-sound-level function at the same frequency , as if deltaphi were caused by a 2-4 dB increase in sound level .
	manualset3
255166	8	423926	15	NULL	NULL	NULL	NULL	frequency	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At tail frequencies , ANF phase changed with sound level ( often by 90 degrees-180 degrees ) and the deltaphi from a fiber was positively correlated with the slope of its phase-versus-sound-level function at the same frequency , as if deltaphi were caused by a 2-4 dB increase in sound level .
	manualset3
255167	9	423926	15	NULL	NULL	NULL	NULL	deltaphi	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At tail frequencies , ANF phase changed with sound level ( often by 90 degrees-180 degrees ) and the deltaphi from a fiber was positively correlated with the slope of its phase-versus-sound-level function at the same frequency , as if deltaphi were caused by a 2-4 dB increase in sound level .
	manualset3
255168	10	423926	15	NULL	NULL	NULL	NULL	2-4 dB	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At tail frequencies , ANF phase changed with sound level ( often by 90 degrees-180 degrees ) and the deltaphi from a fiber was positively correlated with the slope of its phase-versus-sound-level function at the same frequency , as if deltaphi were caused by a 2-4 dB increase in sound level .
	manualset3
255169	11	423926	15	NULL	NULL	NULL	NULL	increase	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At tail frequencies , ANF phase changed with sound level ( often by 90 degrees-180 degrees ) and the deltaphi from a fiber was positively correlated with the slope of its phase-versus-sound-level function at the same frequency , as if deltaphi were caused by a 2-4 dB increase in sound level .
	manualset3
255170	12	423926	15	NULL	NULL	NULL	NULL	sound level	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At tail frequencies , ANF phase changed with sound level ( often by 90 degrees-180 degrees ) and the deltaphi from a fiber was positively correlated with the slope of its phase-versus-sound-level function at the same frequency , as if deltaphi were caused by a 2-4 dB increase in sound level .
	manualset3
255171	1	423927	15	NULL	NULL	NULL	NULL	C-terminal region of the beta barrel	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the C-terminal region of the beta barrel , the Mn2 + and a PEP analog interact with catalytically essential residues , confirmed by site-directed mutagenesis studies .
	manualset3
255172	2	423927	15	NULL	NULL	NULL	NULL	Mn2 +	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the C-terminal region of the beta barrel , the Mn2 + and a PEP analog interact with catalytically essential residues , confirmed by site-directed mutagenesis studies .
	manualset3
255173	3	423927	15	NULL	NULL	NULL	NULL	PEP analog	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the C-terminal region of the beta barrel , the Mn2 + and a PEP analog interact with catalytically essential residues , confirmed by site-directed mutagenesis studies .
	manualset3
255174	4	423927	15	NULL	NULL	NULL	NULL	essential residues	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the C-terminal region of the beta barrel , the Mn2 + and a PEP analog interact with catalytically essential residues , confirmed by site-directed mutagenesis studies .
	manualset3
255175	5	423927	15	NULL	NULL	NULL	NULL	site-directed mutagenesis studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the C-terminal region of the beta barrel , the Mn2 + and a PEP analog interact with catalytically essential residues , confirmed by site-directed mutagenesis studies .
	manualset3
255176	1	423928	15	NULL	NULL	NULL	NULL	Multiple Sclerosis Rehabilitation Hospital	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the Multiple Sclerosis Rehabilitation Hospital , Haslev , 40 patients with mild to moderate cognitive and behavioral impairment associated with MS were randomized to either specific cognitive treatment ( 20 pts ) by direct training , compensatory strategies and neuropsychotherapy , or to non-specific , deliberately diffuse mental stimulation ( 20 pts ) .
	manualset3
255177	2	423928	15	NULL	NULL	NULL	NULL	Haslev	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the Multiple Sclerosis Rehabilitation Hospital , Haslev , 40 patients with mild to moderate cognitive and behavioral impairment associated with MS were randomized to either specific cognitive treatment ( 20 pts ) by direct training , compensatory strategies and neuropsychotherapy , or to non-specific , deliberately diffuse mental stimulation ( 20 pts ) .
	manualset3
255178	3	423928	15	NULL	NULL	NULL	NULL	40 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the Multiple Sclerosis Rehabilitation Hospital , Haslev , 40 patients with mild to moderate cognitive and behavioral impairment associated with MS were randomized to either specific cognitive treatment ( 20 pts ) by direct training , compensatory strategies and neuropsychotherapy , or to non-specific , deliberately diffuse mental stimulation ( 20 pts ) .
	manualset3
255179	4	423928	15	NULL	NULL	NULL	NULL	cognitive impairment 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the Multiple Sclerosis Rehabilitation Hospital , Haslev , 40 patients with mild to moderate cognitive and behavioral impairment associated with MS were randomized to either specific cognitive treatment ( 20 pts ) by direct training , compensatory strategies and neuropsychotherapy , or to non-specific , deliberately diffuse mental stimulation ( 20 pts ) .
	manualset3
255180	5	423928	15	NULL	NULL	NULL	NULL	behavioral impairment 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the Multiple Sclerosis Rehabilitation Hospital , Haslev , 40 patients with mild to moderate cognitive and behavioral impairment associated with MS were randomized to either specific cognitive treatment ( 20 pts ) by direct training , compensatory strategies and neuropsychotherapy , or to non-specific , deliberately diffuse mental stimulation ( 20 pts ) .
	manualset3
255182	6	423928	15	NULL	NULL	NULL	NULL	MS	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the Multiple Sclerosis Rehabilitation Hospital , Haslev , 40 patients with mild to moderate cognitive and behavioral impairment associated with MS were randomized to either specific cognitive treatment ( 20 pts ) by direct training , compensatory strategies and neuropsychotherapy , or to non-specific , deliberately diffuse mental stimulation ( 20 pts ) .
	manualset3
255183	7	423928	15	NULL	NULL	NULL	NULL	specific cognitive treatment 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the Multiple Sclerosis Rehabilitation Hospital , Haslev , 40 patients with mild to moderate cognitive and behavioral impairment associated with MS were randomized to either specific cognitive treatment ( 20 pts ) by direct training , compensatory strategies and neuropsychotherapy , or to non-specific , deliberately diffuse mental stimulation ( 20 pts ) .
	manualset3
255184	8	423928	15	NULL	NULL	NULL	NULL	20 pts 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the Multiple Sclerosis Rehabilitation Hospital , Haslev , 40 patients with mild to moderate cognitive and behavioral impairment associated with MS were randomized to either specific cognitive treatment ( 20 pts ) by direct training , compensatory strategies and neuropsychotherapy , or to non-specific , deliberately diffuse mental stimulation ( 20 pts ) .
	manualset3
255185	9	423928	15	NULL	NULL	NULL	NULL	direct training	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the Multiple Sclerosis Rehabilitation Hospital , Haslev , 40 patients with mild to moderate cognitive and behavioral impairment associated with MS were randomized to either specific cognitive treatment ( 20 pts ) by direct training , compensatory strategies and neuropsychotherapy , or to non-specific , deliberately diffuse mental stimulation ( 20 pts ) .
	manualset3
255187	10	423928	15	NULL	NULL	NULL	NULL	compensatory strategies	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the Multiple Sclerosis Rehabilitation Hospital , Haslev , 40 patients with mild to moderate cognitive and behavioral impairment associated with MS were randomized to either specific cognitive treatment ( 20 pts ) by direct training , compensatory strategies and neuropsychotherapy , or to non-specific , deliberately diffuse mental stimulation ( 20 pts ) .
	manualset3
255188	11	423928	15	NULL	NULL	NULL	NULL	neuropsychotherapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the Multiple Sclerosis Rehabilitation Hospital , Haslev , 40 patients with mild to moderate cognitive and behavioral impairment associated with MS were randomized to either specific cognitive treatment ( 20 pts ) by direct training , compensatory strategies and neuropsychotherapy , or to non-specific , deliberately diffuse mental stimulation ( 20 pts ) .
	manualset3
255189	12	423928	15	NULL	NULL	NULL	NULL	diffuse mental stimulation 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the Multiple Sclerosis Rehabilitation Hospital , Haslev , 40 patients with mild to moderate cognitive and behavioral impairment associated with MS were randomized to either specific cognitive treatment ( 20 pts ) by direct training , compensatory strategies and neuropsychotherapy , or to non-specific , deliberately diffuse mental stimulation ( 20 pts ) .
	manualset3
255190	13	423928	15	NULL	NULL	NULL	NULL	20 pts 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the Multiple Sclerosis Rehabilitation Hospital , Haslev , 40 patients with mild to moderate cognitive and behavioral impairment associated with MS were randomized to either specific cognitive treatment ( 20 pts ) by direct training , compensatory strategies and neuropsychotherapy , or to non-specific , deliberately diffuse mental stimulation ( 20 pts ) .
	manualset3
255191	1	423929	15	NULL	NULL	NULL	NULL	age of 2 months	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the age of 2 months the src ( - / - ) mice presented signs of airway obstruction and all mice died progressively between 2.5 and 6 months of age .
	manualset3
255192	2	423929	15	NULL	NULL	NULL	NULL	src ( - / - ) mice	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the age of 2 months the src ( - / - ) mice presented signs of airway obstruction and all mice died progressively between 2.5 and 6 months of age .
	manualset3
255193	3	423929	15	NULL	NULL	NULL	NULL	signs of airway obstruction	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the age of 2 months the src ( - / - ) mice presented signs of airway obstruction and all mice died progressively between 2.5 and 6 months of age .
	manualset3
255194	4	423929	15	NULL	NULL	NULL	NULL	mice 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the age of 2 months the src ( - / - ) mice presented signs of airway obstruction and all mice died progressively between 2.5 and 6 months of age .
	manualset3
255195	5	423929	15	NULL	NULL	NULL	NULL	2.5 and 6 months of age	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the age of 2 months the src ( - / - ) mice presented signs of airway obstruction and all mice died progressively between 2.5 and 6 months of age .
	manualset3
255249	1	423930	15	NULL	NULL	NULL	NULL	age of 7 weeks	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the age of 7 or 17 weeks , SBP and ( Ca2 + ) i of SHRSP were significantly higher than in WKY , and at the age of 17 weeks , ( Mg2 + ) i of SHRSP was significantly lower than in WKY .
	manualset3
255250	2	423930	15	NULL	NULL	NULL	NULL	age of 17 weeks	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the age of 7 or 17 weeks , SBP and ( Ca2 + ) i of SHRSP were significantly higher than in WKY , and at the age of 17 weeks , ( Mg2 + ) i of SHRSP was significantly lower than in WKY .
	manualset3
255251	3	423930	15	NULL	NULL	NULL	NULL	SBP 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the age of 7 or 17 weeks , SBP and ( Ca2 + ) i of SHRSP were significantly higher than in WKY , and at the age of 17 weeks , ( Mg2 + ) i of SHRSP was significantly lower than in WKY .
	manualset3
255252	4	423930	15	NULL	NULL	NULL	NULL	( Ca2 + ) i 	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the age of 7 or 17 weeks , SBP and ( Ca2 + ) i of SHRSP were significantly higher than in WKY , and at the age of 17 weeks , ( Mg2 + ) i of SHRSP was significantly lower than in WKY .
	manualset3
255253	5	423930	15	NULL	NULL	NULL	NULL	SHRSP	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the age of 7 or 17 weeks , SBP and ( Ca2 + ) i of SHRSP were significantly higher than in WKY , and at the age of 17 weeks , ( Mg2 + ) i of SHRSP was significantly lower than in WKY .
	manualset3
255254	6	423930	15	NULL	NULL	NULL	NULL	WKY	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the age of 7 or 17 weeks , SBP and ( Ca2 + ) i of SHRSP were significantly higher than in WKY , and at the age of 17 weeks , ( Mg2 + ) i of SHRSP was significantly lower than in WKY .
	manualset3
255256	7	423930	15	NULL	NULL	NULL	NULL	age of 17 weeks	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the age of 7 or 17 weeks , SBP and ( Ca2 + ) i of SHRSP were significantly higher than in WKY , and at the age of 17 weeks , ( Mg2 + ) i of SHRSP was significantly lower than in WKY .
	manualset3
255257	8	423930	15	NULL	NULL	NULL	NULL	( Mg2 + ) i	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the age of 7 or 17 weeks , SBP and ( Ca2 + ) i of SHRSP were significantly higher than in WKY , and at the age of 17 weeks , ( Mg2 + ) i of SHRSP was significantly lower than in WKY .
	manualset3
255258	9	423930	15	NULL	NULL	NULL	NULL	SHRSP	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the age of 7 or 17 weeks , SBP and ( Ca2 + ) i of SHRSP were significantly higher than in WKY , and at the age of 17 weeks , ( Mg2 + ) i of SHRSP was significantly lower than in WKY .
	manualset3
255259	10	423930	15	NULL	NULL	NULL	NULL	WKY	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the age of 7 or 17 weeks , SBP and ( Ca2 + ) i of SHRSP were significantly higher than in WKY , and at the age of 17 weeks , ( Mg2 + ) i of SHRSP was significantly lower than in WKY .
	manualset3
255290	1	423931	15	NULL	NULL	NULL	NULL	base of the column 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the base of the column are Merkel cell complexes , known to be type I slowly adapting mechanoreceptors , and lamellated corpuscles , probably vibration receptors .
	manualset3
255291	2	423931	15	NULL	NULL	NULL	NULL	Merkel cell complexes 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the base of the column are Merkel cell complexes , known to be type I slowly adapting mechanoreceptors , and lamellated corpuscles , probably vibration receptors .
	manualset3
255292	3	423931	15	NULL	NULL	NULL	NULL	type I slowly adapting mechanoreceptors 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the base of the column are Merkel cell complexes , known to be type I slowly adapting mechanoreceptors , and lamellated corpuscles , probably vibration receptors .
	manualset3
255293	4	423931	15	NULL	NULL	NULL	NULL	lamellated corpuscles	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the base of the column are Merkel cell complexes , known to be type I slowly adapting mechanoreceptors , and lamellated corpuscles , probably vibration receptors .
	manualset3
255294	5	423931	15	NULL	NULL	NULL	NULL	vibration receptors	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the base of the column are Merkel cell complexes , known to be type I slowly adapting mechanoreceptors , and lamellated corpuscles , probably vibration receptors .
	manualset3
255295	1	423932	15	NULL	NULL	NULL	NULL	beginning of the trial year	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the beginning and the end of the trial year , households surveys were conducted in the catchment areas of the health centres , and focus group discussions with pregnant women and mothers of children under 5 years were conducted .
	manualset3
255300	2	423932	15	NULL	NULL	NULL	NULL	end of the trial year	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the beginning and the end of the trial year , households surveys were conducted in the catchment areas of the health centres , and focus group discussions with pregnant women and mothers of children under 5 years were conducted .
	manualset3
255301	3	423932	15	NULL	NULL	NULL	NULL	households surveys	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the beginning and the end of the trial year , households surveys were conducted in the catchment areas of the health centres , and focus group discussions with pregnant women and mothers of children under 5 years were conducted .
	manualset3
255302	4	423932	15	NULL	NULL	NULL	NULL	catchment areas	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the beginning and the end of the trial year , households surveys were conducted in the catchment areas of the health centres , and focus group discussions with pregnant women and mothers of children under 5 years were conducted .
	manualset3
255304	5	423932	15	NULL	NULL	NULL	NULL	health centres	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the beginning and the end of the trial year , households surveys were conducted in the catchment areas of the health centres , and focus group discussions with pregnant women and mothers of children under 5 years were conducted .
	manualset3
255305	6	423932	15	NULL	NULL	NULL	NULL	focus group discussions	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the beginning and the end of the trial year , households surveys were conducted in the catchment areas of the health centres , and focus group discussions with pregnant women and mothers of children under 5 years were conducted .
	manualset3
255306	7	423932	15	NULL	NULL	NULL	NULL	pregnant women	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the beginning and the end of the trial year , households surveys were conducted in the catchment areas of the health centres , and focus group discussions with pregnant women and mothers of children under 5 years were conducted .
	manualset3
255307	8	423932	15	NULL	NULL	NULL	NULL	mothers of children under 5 years	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the beginning and the end of the trial year , households surveys were conducted in the catchment areas of the health centres , and focus group discussions with pregnant women and mothers of children under 5 years were conducted .
	manualset3
255289	1	423933	15	NULL	NULL	NULL	NULL	beginning of 2002	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the beginning of 2002 , some Thai shrimp farmers complained that ponds stocked with WSSV-232 PCR negative post-larvae ( PL ) later suffered WSSV disease outbreaks .
	manualset3
255296	2	423933	15	NULL	NULL	NULL	NULL	Thai shrimp farmers	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the beginning of 2002 , some Thai shrimp farmers complained that ponds stocked with WSSV-232 PCR negative post-larvae ( PL ) later suffered WSSV disease outbreaks .
	manualset3
255297	3	423933	15	NULL	NULL	NULL	NULL	ponds 	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the beginning of 2002 , some Thai shrimp farmers complained that ponds stocked with WSSV-232 PCR negative post-larvae ( PL ) later suffered WSSV disease outbreaks .
	manualset3
255298	4	423933	15	NULL	NULL	NULL	NULL	WSSV-232 PCR negative post-larvae ( PL ) 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the beginning of 2002 , some Thai shrimp farmers complained that ponds stocked with WSSV-232 PCR negative post-larvae ( PL ) later suffered WSSV disease outbreaks .
	manualset3
255299	5	423933	15	NULL	NULL	NULL	NULL	WSSV disease outbreaks 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the beginning of 2002 , some Thai shrimp farmers complained that ponds stocked with WSSV-232 PCR negative post-larvae ( PL ) later suffered WSSV disease outbreaks .
	manualset3
255308	1	423934	15	NULL	NULL	NULL	NULL	beginning of eighteen century ( 18th )	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the beginning of eighteen century ( 18th ) , morphine was used for the first time in analgesic aim .
	manualset3
255309	2	423934	15	NULL	NULL	NULL	NULL	morphine 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the beginning of eighteen century ( 18th ) , morphine was used for the first time in analgesic aim .
	manualset3
255310	3	423934	15	NULL	NULL	NULL	NULL	time	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the beginning of eighteen century ( 18th ) , morphine was used for the first time in analgesic aim .
	manualset3
255311	4	423934	15	NULL	NULL	NULL	NULL	analgesic aim	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the beginning of eighteen century ( 18th ) , morphine was used for the first time in analgesic aim .
	manualset3
255312	1	423935	15	NULL	NULL	NULL	NULL	comparative study 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( A comparative study of the morphology of the Trypanosoma brucei brucei trypomastigote using photonic microscopy and scanning electron microscopy ( author 's transl ) ) .
	manualset3
255462	2	423935	15	NULL	NULL	NULL	NULL	morphology 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( A comparative study of the morphology of the Trypanosoma brucei brucei trypomastigote using photonic microscopy and scanning electron microscopy ( author 's transl ) ) .
	manualset3
255465	3	423935	15	NULL	NULL	NULL	NULL	Trypanosoma brucei brucei trypomastigote 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( A comparative study of the morphology of the Trypanosoma brucei brucei trypomastigote using photonic microscopy and scanning electron microscopy ( author 's transl ) ) .
	manualset3
255468	4	423935	15	NULL	NULL	NULL	NULL	photonic microscopy	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( A comparative study of the morphology of the Trypanosoma brucei brucei trypomastigote using photonic microscopy and scanning electron microscopy ( author 's transl ) ) .
	manualset3
255471	5	423935	15	NULL	NULL	NULL	NULL	scanning electron microscopy	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( A comparative study of the morphology of the Trypanosoma brucei brucei trypomastigote using photonic microscopy and scanning electron microscopy ( author 's transl ) ) .
	manualset3
255473	6	423935	15	NULL	NULL	NULL	NULL	author 's transl 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( A comparative study of the morphology of the Trypanosoma brucei brucei trypomastigote using photonic microscopy and scanning electron microscopy ( author 's transl ) ) .
	manualset3
255314	1	423936	15	NULL	NULL	NULL	NULL	Epiphysiolysis capitis femoris	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Epiphysiolysis capitis femoris in a horse ) .
	manualset3
255317	2	423936	15	NULL	NULL	NULL	NULL	horse	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Epiphysiolysis capitis femoris in a horse ) .
	manualset3
255318	1	423937	15	NULL	NULL	NULL	NULL	earliest times 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the earliest times examined after infection , the HSV-1 genome is incorporated into chromatin that predominantly contains the variant H3 .3 , whereas incorporation of canonical H3 .1 occurs later in infection and is dependent on replication of the HSV-1 genome .
	manualset3
255319	2	423937	15	NULL	NULL	NULL	NULL	infection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the earliest times examined after infection , the HSV-1 genome is incorporated into chromatin that predominantly contains the variant H3 .3 , whereas incorporation of canonical H3 .1 occurs later in infection and is dependent on replication of the HSV-1 genome .
	manualset3
255320	3	423937	15	NULL	NULL	NULL	NULL	HSV-1 genome	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the earliest times examined after infection , the HSV-1 genome is incorporated into chromatin that predominantly contains the variant H3 .3 , whereas incorporation of canonical H3 .1 occurs later in infection and is dependent on replication of the HSV-1 genome .
	manualset3
255321	4	423937	15	NULL	NULL	NULL	NULL	chromatin	Chromosome												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the earliest times examined after infection , the HSV-1 genome is incorporated into chromatin that predominantly contains the variant H3 .3 , whereas incorporation of canonical H3 .1 occurs later in infection and is dependent on replication of the HSV-1 genome .
	manualset3
255322	5	423937	15	NULL	NULL	NULL	NULL	variant H3 .3	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the earliest times examined after infection , the HSV-1 genome is incorporated into chromatin that predominantly contains the variant H3 .3 , whereas incorporation of canonical H3 .1 occurs later in infection and is dependent on replication of the HSV-1 genome .
	manualset3
255323	6	423937	15	NULL	NULL	NULL	NULL	incorporation of canonical H3 .1 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the earliest times examined after infection , the HSV-1 genome is incorporated into chromatin that predominantly contains the variant H3 .3 , whereas incorporation of canonical H3 .1 occurs later in infection and is dependent on replication of the HSV-1 genome .
	manualset3
255324	7	423937	15	NULL	NULL	NULL	NULL	infection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the earliest times examined after infection , the HSV-1 genome is incorporated into chromatin that predominantly contains the variant H3 .3 , whereas incorporation of canonical H3 .1 occurs later in infection and is dependent on replication of the HSV-1 genome .
	manualset3
255325	8	423937	15	NULL	NULL	NULL	NULL	replication of the HSV-1 genome 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the earliest times examined after infection , the HSV-1 genome is incorporated into chromatin that predominantly contains the variant H3 .3 , whereas incorporation of canonical H3 .1 occurs later in infection and is dependent on replication of the HSV-1 genome .
	manualset3
255326	1	423938	15	NULL	NULL	NULL	NULL	end of the 4th week 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of the 4th week , both serum albumin ( 3.90 + / - 0.31 g/dl ) and prealbumin ( 27.33 + / - 3.30 mg/dl ) in experimental group returned to normal , being also significantly higher than those in the control group ( 3.00 + / - 0.23 g/dl , P & lt ; 0.05 ; 17.11 + / - 3.22 mg/dl , P & lt ; 0.01 ) .
	manualset3
255327	2	423938	15	NULL	NULL	NULL	NULL	serum albumin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of the 4th week , both serum albumin ( 3.90 + / - 0.31 g/dl ) and prealbumin ( 27.33 + / - 3.30 mg/dl ) in experimental group returned to normal , being also significantly higher than those in the control group ( 3.00 + / - 0.23 g/dl , P & lt ; 0.05 ; 17.11 + / - 3.22 mg/dl , P & lt ; 0.01 ) .
	manualset3
255328	3	423938	15	NULL	NULL	NULL	NULL	3.90 + / - 0.31 g/dl	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of the 4th week , both serum albumin ( 3.90 + / - 0.31 g/dl ) and prealbumin ( 27.33 + / - 3.30 mg/dl ) in experimental group returned to normal , being also significantly higher than those in the control group ( 3.00 + / - 0.23 g/dl , P & lt ; 0.05 ; 17.11 + / - 3.22 mg/dl , P & lt ; 0.01 ) .
	manualset3
255478	4	423938	15	NULL	NULL	NULL	NULL	prealbumin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of the 4th week , both serum albumin ( 3.90 + / - 0.31 g/dl ) and prealbumin ( 27.33 + / - 3.30 mg/dl ) in experimental group returned to normal , being also significantly higher than those in the control group ( 3.00 + / - 0.23 g/dl , P & lt ; 0.05 ; 17.11 + / - 3.22 mg/dl , P & lt ; 0.01 ) .
	manualset3
255480	5	423938	15	NULL	NULL	NULL	NULL	27.33 + / - 3.30 mg/dl 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of the 4th week , both serum albumin ( 3.90 + / - 0.31 g/dl ) and prealbumin ( 27.33 + / - 3.30 mg/dl ) in experimental group returned to normal , being also significantly higher than those in the control group ( 3.00 + / - 0.23 g/dl , P & lt ; 0.05 ; 17.11 + / - 3.22 mg/dl , P & lt ; 0.01 ) .
	manualset3
255485	6	423938	15	NULL	NULL	NULL	NULL	experimental group	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of the 4th week , both serum albumin ( 3.90 + / - 0.31 g/dl ) and prealbumin ( 27.33 + / - 3.30 mg/dl ) in experimental group returned to normal , being also significantly higher than those in the control group ( 3.00 + / - 0.23 g/dl , P & lt ; 0.05 ; 17.11 + / - 3.22 mg/dl , P & lt ; 0.01 ) .
	manualset3
255491	7	423938	15	NULL	NULL	NULL	NULL	control group	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of the 4th week , both serum albumin ( 3.90 + / - 0.31 g/dl ) and prealbumin ( 27.33 + / - 3.30 mg/dl ) in experimental group returned to normal , being also significantly higher than those in the control group ( 3.00 + / - 0.23 g/dl , P & lt ; 0.05 ; 17.11 + / - 3.22 mg/dl , P & lt ; 0.01 ) .
	manualset3
255493	8	423938	15	NULL	NULL	NULL	NULL	3.00 + / - 0.23 g/dl	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of the 4th week , both serum albumin ( 3.90 + / - 0.31 g/dl ) and prealbumin ( 27.33 + / - 3.30 mg/dl ) in experimental group returned to normal , being also significantly higher than those in the control group ( 3.00 + / - 0.23 g/dl , P & lt ; 0.05 ; 17.11 + / - 3.22 mg/dl , P & lt ; 0.01 ) .
	manualset3
255495	9	423938	15	NULL	NULL	NULL	NULL	P & lt ; 0.05	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of the 4th week , both serum albumin ( 3.90 + / - 0.31 g/dl ) and prealbumin ( 27.33 + / - 3.30 mg/dl ) in experimental group returned to normal , being also significantly higher than those in the control group ( 3.00 + / - 0.23 g/dl , P & lt ; 0.05 ; 17.11 + / - 3.22 mg/dl , P & lt ; 0.01 ) .
	manualset3
255496	10	423938	15	NULL	NULL	NULL	NULL	17.11 + / - 3.22 mg/dl 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of the 4th week , both serum albumin ( 3.90 + / - 0.31 g/dl ) and prealbumin ( 27.33 + / - 3.30 mg/dl ) in experimental group returned to normal , being also significantly higher than those in the control group ( 3.00 + / - 0.23 g/dl , P & lt ; 0.05 ; 17.11 + / - 3.22 mg/dl , P & lt ; 0.01 ) .
	manualset3
255499	11	423938	15	NULL	NULL	NULL	NULL	P & lt ; 0.01	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of the 4th week , both serum albumin ( 3.90 + / - 0.31 g/dl ) and prealbumin ( 27.33 + / - 3.30 mg/dl ) in experimental group returned to normal , being also significantly higher than those in the control group ( 3.00 + / - 0.23 g/dl , P & lt ; 0.05 ; 17.11 + / - 3.22 mg/dl , P & lt ; 0.01 ) .
	manualset3
255508	1	423939	15	NULL	NULL	NULL	NULL	end	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of the procedure , animals were sacrificed for histological study .
	manualset3
255511	3	423939	15	NULL	NULL	NULL	NULL	animals	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of the procedure , animals were sacrificed for histological study .
	manualset3
255513	4	423939	15	NULL	NULL	NULL	NULL	histological study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of the procedure , animals were sacrificed for histological study .
	manualset3
255522	2	423939	15	NULL	NULL	NULL	NULL	procedure	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of the procedure , animals were sacrificed for histological study .
	manualset3
255530	1	423940	15	NULL	NULL	NULL	NULL	end 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of the semester , student perceptions and course performance were examined .
	manualset3
255531	2	423940	15	NULL	NULL	NULL	NULL	semester	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of the semester , student perceptions and course performance were examined .
	manualset3
255535	3	423940	15	NULL	NULL	NULL	NULL	student perceptions	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of the semester , student perceptions and course performance were examined .
	manualset3
255539	4	423940	15	NULL	NULL	NULL	NULL	course performance	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of the semester , student perceptions and course performance were examined .
	manualset3
255545	1	423941	15	NULL	NULL	NULL	NULL	end 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of the stimulation , the environment of the animals became stationary , but the eye did not immediately return to a fixed stable position .
	manualset3
255547	2	423941	15	NULL	NULL	NULL	NULL	stimulation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of the stimulation , the environment of the animals became stationary , but the eye did not immediately return to a fixed stable position .
	manualset3
255548	3	423941	15	NULL	NULL	NULL	NULL	environment of the animals	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of the stimulation , the environment of the animals became stationary , but the eye did not immediately return to a fixed stable position .
	manualset3
255549	4	423941	15	NULL	NULL	NULL	NULL	eye 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of the stimulation , the environment of the animals became stationary , but the eye did not immediately return to a fixed stable position .
	manualset3
255551	5	423941	15	NULL	NULL	NULL	NULL	fixed stable position 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of the stimulation , the environment of the animals became stationary , but the eye did not immediately return to a fixed stable position .
	manualset3
255555	1	423942	15	NULL	NULL	NULL	NULL	end	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of treatment 66 % of the patients in the haloperidol group and 22 % in the remoxipride group were using anticholinergics .
	manualset3
255559	2	423942	15	NULL	NULL	NULL	NULL	treatment 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of treatment 66 % of the patients in the haloperidol group and 22 % in the remoxipride group were using anticholinergics .
	manualset3
255560	3	423942	15	NULL	NULL	NULL	NULL	66 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of treatment 66 % of the patients in the haloperidol group and 22 % in the remoxipride group were using anticholinergics .
	manualset3
255562	4	423942	15	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of treatment 66 % of the patients in the haloperidol group and 22 % in the remoxipride group were using anticholinergics .
	manualset3
255564	5	423942	15	NULL	NULL	NULL	NULL	haloperidol group	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of treatment 66 % of the patients in the haloperidol group and 22 % in the remoxipride group were using anticholinergics .
	manualset3
255566	6	423942	15	NULL	NULL	NULL	NULL	22 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of treatment 66 % of the patients in the haloperidol group and 22 % in the remoxipride group were using anticholinergics .
	manualset3
255567	7	423942	15	NULL	NULL	NULL	NULL	remoxipride group	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of treatment 66 % of the patients in the haloperidol group and 22 % in the remoxipride group were using anticholinergics .
	manualset3
255568	8	423942	15	NULL	NULL	NULL	NULL	anticholinergics	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the end of treatment 66 % of the patients in the haloperidol group and 22 % in the remoxipride group were using anticholinergics .
	manualset3
255576	1	423943	15	NULL	NULL	NULL	NULL	Errors	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Errors in the comparative evaluation of complex indices of atmospheric air pollution ) .
	manualset3
255578	2	423943	15	NULL	NULL	NULL	NULL	comparative evaluation of complex indices 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Errors in the comparative evaluation of complex indices of atmospheric air pollution ) .
	manualset3
255579	3	423943	15	NULL	NULL	NULL	NULL	atmospheric air pollution	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Errors in the comparative evaluation of complex indices of atmospheric air pollution ) .
	manualset3
255580	1	423944	15	NULL	NULL	NULL	NULL	expense of complexity	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the expense of complexity , average system performance is shown to be significantly better than that of several known comparison systems , particularly at higher channel bit error rates .
	manualset3
255582	2	423944	15	NULL	NULL	NULL	NULL	average system performance	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the expense of complexity , average system performance is shown to be significantly better than that of several known comparison systems , particularly at higher channel bit error rates .
	manualset3
255583	3	423944	15	NULL	NULL	NULL	NULL	comparison systems 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the expense of complexity , average system performance is shown to be significantly better than that of several known comparison systems , particularly at higher channel bit error rates .
	manualset3
255584	4	423944	15	NULL	NULL	NULL	NULL	channel bit error rates	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the expense of complexity , average system performance is shown to be significantly better than that of several known comparison systems , particularly at higher channel bit error rates .
	manualset3
255590	1	423945	15	NULL	NULL	NULL	NULL	first step	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the first step , we compared the blood concentration of fentanyl in the azygos vein after thoracic epidural and that after caudal administration .
	manualset3
255594	2	423945	15	NULL	NULL	NULL	NULL	blood concentration	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the first step , we compared the blood concentration of fentanyl in the azygos vein after thoracic epidural and that after caudal administration .
	manualset3
255595	3	423945	15	NULL	NULL	NULL	NULL	fentanyl	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the first step , we compared the blood concentration of fentanyl in the azygos vein after thoracic epidural and that after caudal administration .
	manualset3
255596	4	423945	15	NULL	NULL	NULL	NULL	azygos vein 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the first step , we compared the blood concentration of fentanyl in the azygos vein after thoracic epidural and that after caudal administration .
	manualset3
255599	5	423945	15	NULL	NULL	NULL	NULL	thoracic epidural administration	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the first step , we compared the blood concentration of fentanyl in the azygos vein after thoracic epidural and that after caudal administration .
	manualset3
255602	6	423945	15	NULL	NULL	NULL	NULL	caudal administration	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the first step , we compared the blood concentration of fentanyl in the azygos vein after thoracic epidural and that after caudal administration .
	manualset3
255606	1	423946	15	NULL	NULL	NULL	NULL	girl scout camp	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the girl scout camp , exposure both within and between activity groups varied substantially and were more variable than the baseball players ' exposure .
	manualset3
255607	2	423946	15	NULL	NULL	NULL	NULL	exposure 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the girl scout camp , exposure both within and between activity groups varied substantially and were more variable than the baseball players ' exposure .
	manualset3
255609	3	423946	15	NULL	NULL	NULL	NULL	activity groups	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the girl scout camp , exposure both within and between activity groups varied substantially and were more variable than the baseball players ' exposure .
	manualset3
255623	4	423946	15	NULL	NULL	NULL	NULL	baseball players ' exposure	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the girl scout camp , exposure both within and between activity groups varied substantially and were more variable than the baseball players ' exposure .
	manualset3
255630	1	423947	15	NULL	NULL	NULL	NULL	applied shear rates 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the highest applied shear rates of 408 and 510 s-1 , the initial adsorption rate of fibrinogen was estimated to be 5.0 X 10 ( -5 ) cm/s on both surfaces .
	manualset3
255641	2	423947	15	NULL	NULL	NULL	NULL	408 s-1	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the highest applied shear rates of 408 and 510 s-1 , the initial adsorption rate of fibrinogen was estimated to be 5.0 X 10 ( -5 ) cm/s on both surfaces .
	manualset3
255642	3	423947	15	NULL	NULL	NULL	NULL	510 s-1	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the highest applied shear rates of 408 and 510 s-1 , the initial adsorption rate of fibrinogen was estimated to be 5.0 X 10 ( -5 ) cm/s on both surfaces .
	manualset3
255645	4	423947	15	NULL	NULL	NULL	NULL	initial adsorption rate	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the highest applied shear rates of 408 and 510 s-1 , the initial adsorption rate of fibrinogen was estimated to be 5.0 X 10 ( -5 ) cm/s on both surfaces .
	manualset3
255647	5	423947	15	NULL	NULL	NULL	NULL	fibrinogen 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the highest applied shear rates of 408 and 510 s-1 , the initial adsorption rate of fibrinogen was estimated to be 5.0 X 10 ( -5 ) cm/s on both surfaces .
	manualset3
255649	6	423947	15	NULL	NULL	NULL	NULL	5.0 X 10 ( -5 ) cm/s	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the highest applied shear rates of 408 and 510 s-1 , the initial adsorption rate of fibrinogen was estimated to be 5.0 X 10 ( -5 ) cm/s on both surfaces .
	manualset3
255650	7	423947	15	NULL	NULL	NULL	NULL	surfaces	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the highest applied shear rates of 408 and 510 s-1 , the initial adsorption rate of fibrinogen was estimated to be 5.0 X 10 ( -5 ) cm/s on both surfaces .
	manualset3
255656	1	423948	15	NULL	NULL	NULL	NULL	initial procedure	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the initial procedure , the lateral crura are positioned and a tiny biconcave prolabium is shaped in anticipation of the changes with growth .
	manualset3
255663	2	423948	15	NULL	NULL	NULL	NULL	lateral crura	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the initial procedure , the lateral crura are positioned and a tiny biconcave prolabium is shaped in anticipation of the changes with growth .
	manualset3
255664	3	423948	15	NULL	NULL	NULL	NULL	tiny biconcave prolabium	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the initial procedure , the lateral crura are positioned and a tiny biconcave prolabium is shaped in anticipation of the changes with growth .
	manualset3
255667	4	423948	15	NULL	NULL	NULL	NULL	anticipation	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the initial procedure , the lateral crura are positioned and a tiny biconcave prolabium is shaped in anticipation of the changes with growth .
	manualset3
255670	5	423948	15	NULL	NULL	NULL	NULL	changes 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the initial procedure , the lateral crura are positioned and a tiny biconcave prolabium is shaped in anticipation of the changes with growth .
	manualset3
255671	6	423948	15	NULL	NULL	NULL	NULL	growth	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the initial procedure , the lateral crura are positioned and a tiny biconcave prolabium is shaped in anticipation of the changes with growth .
	manualset3
255680	1	423949	15	NULL	NULL	NULL	NULL	ovary	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the level of the ovary , the prostaglandins E may be modulators of the action of gonadostimulin on ovarian hormonogenesis , in close relationship with cyclic AMP and , furthermore , represent an important biochemical intermediate stage in the mechanism of ovulation .
	manualset3
255681	2	423949	15	NULL	NULL	NULL	NULL	prostaglandins E	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the level of the ovary , the prostaglandins E may be modulators of the action of gonadostimulin on ovarian hormonogenesis , in close relationship with cyclic AMP and , furthermore , represent an important biochemical intermediate stage in the mechanism of ovulation .
	manualset3
255682	3	423949	15	NULL	NULL	NULL	NULL	modulators	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the level of the ovary , the prostaglandins E may be modulators of the action of gonadostimulin on ovarian hormonogenesis , in close relationship with cyclic AMP and , furthermore , represent an important biochemical intermediate stage in the mechanism of ovulation .
	manualset3
255683	4	423949	15	NULL	NULL	NULL	NULL	action of gonadostimulin	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the level of the ovary , the prostaglandins E may be modulators of the action of gonadostimulin on ovarian hormonogenesis , in close relationship with cyclic AMP and , furthermore , represent an important biochemical intermediate stage in the mechanism of ovulation .
	manualset3
255684	5	423949	15	NULL	NULL	NULL	NULL	ovarian hormonogenesis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the level of the ovary , the prostaglandins E may be modulators of the action of gonadostimulin on ovarian hormonogenesis , in close relationship with cyclic AMP and , furthermore , represent an important biochemical intermediate stage in the mechanism of ovulation .
	manualset3
255685	6	423949	15	NULL	NULL	NULL	NULL	relationship	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the level of the ovary , the prostaglandins E may be modulators of the action of gonadostimulin on ovarian hormonogenesis , in close relationship with cyclic AMP and , furthermore , represent an important biochemical intermediate stage in the mechanism of ovulation .
	manualset3
255686	7	423949	15	NULL	NULL	NULL	NULL	cyclic AMP	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the level of the ovary , the prostaglandins E may be modulators of the action of gonadostimulin on ovarian hormonogenesis , in close relationship with cyclic AMP and , furthermore , represent an important biochemical intermediate stage in the mechanism of ovulation .
	manualset3
255687	8	423949	15	NULL	NULL	NULL	NULL	biochemical intermediate stage 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the level of the ovary , the prostaglandins E may be modulators of the action of gonadostimulin on ovarian hormonogenesis , in close relationship with cyclic AMP and , furthermore , represent an important biochemical intermediate stage in the mechanism of ovulation .
	manualset3
255688	9	423949	15	NULL	NULL	NULL	NULL	mechanism of ovulation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the level of the ovary , the prostaglandins E may be modulators of the action of gonadostimulin on ovarian hormonogenesis , in close relationship with cyclic AMP and , furthermore , represent an important biochemical intermediate stage in the mechanism of ovulation .
	manualset3
255689	1	423950	15	NULL	NULL	NULL	NULL	light microscopic level	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the light microscopic level , the Kv1 .4 subunit showed a unique distribution pattern , being localized in specific neuronal populations of the rat brain .
	manualset3
255690	2	423950	15	NULL	NULL	NULL	NULL	Kv1 .4 subunit	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the light microscopic level , the Kv1 .4 subunit showed a unique distribution pattern , being localized in specific neuronal populations of the rat brain .
	manualset3
255691	3	423950	15	NULL	NULL	NULL	NULL	unique distribution pattern	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the light microscopic level , the Kv1 .4 subunit showed a unique distribution pattern , being localized in specific neuronal populations of the rat brain .
	manualset3
255692	4	423950	15	NULL	NULL	NULL	NULL	neuronal population	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the light microscopic level , the Kv1 .4 subunit showed a unique distribution pattern , being localized in specific neuronal populations of the rat brain .
	manualset3
255693	5	423950	15	NULL	NULL	NULL	NULL	rat brain	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the light microscopic level , the Kv1 .4 subunit showed a unique distribution pattern , being localized in specific neuronal populations of the rat brain .
	manualset3
255694	1	423951	15	NULL	NULL	NULL	NULL	concentration range	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the low concentration range , uptake rate was similar for arsenate and arsenite , but at the high concentration range , arsenite was taken up at a faster rate .
	manualset3
255695	2	423951	15	NULL	NULL	NULL	NULL	uptake rate	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the low concentration range , uptake rate was similar for arsenate and arsenite , but at the high concentration range , arsenite was taken up at a faster rate .
	manualset3
255696	3	423951	15	NULL	NULL	NULL	NULL	arsenate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the low concentration range , uptake rate was similar for arsenate and arsenite , but at the high concentration range , arsenite was taken up at a faster rate .
	manualset3
255697	4	423951	15	NULL	NULL	NULL	NULL	arsenite	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the low concentration range , uptake rate was similar for arsenate and arsenite , but at the high concentration range , arsenite was taken up at a faster rate .
	manualset3
255698	5	423951	15	NULL	NULL	NULL	NULL	concentration range	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the low concentration range , uptake rate was similar for arsenate and arsenite , but at the high concentration range , arsenite was taken up at a faster rate .
	manualset3
255699	6	423951	15	NULL	NULL	NULL	NULL	arsenite 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the low concentration range , uptake rate was similar for arsenate and arsenite , but at the high concentration range , arsenite was taken up at a faster rate .
	manualset3
255700	7	423951	15	NULL	NULL	NULL	NULL	rate	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the low concentration range , uptake rate was similar for arsenate and arsenite , but at the high concentration range , arsenite was taken up at a faster rate .
	manualset3
255701	1	423952	15	NULL	NULL	NULL	NULL	Erythrocyte count	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Erythrocyte count during the course of nephropathies ) .
	manualset3
255702	2	423952	15	NULL	NULL	NULL	NULL	course of nephropathies	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Erythrocyte count during the course of nephropathies ) .
	manualset3
255703	1	423953	15	NULL	NULL	NULL	NULL	temperature	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the permissive temperature , smc5-31 but not smc5-33 cells exhibit hypersensitivity to several DNA-damaging agents despite induction of the DNA damage checkpoint .
	manualset3
255966	2	423953	15	NULL	NULL	NULL	NULL	smc5-31 cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the permissive temperature , smc5-31 but not smc5-33 cells exhibit hypersensitivity to several DNA-damaging agents despite induction of the DNA damage checkpoint .
	manualset3
255967	3	423953	15	NULL	NULL	NULL	NULL	smc5-33 cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the permissive temperature , smc5-31 but not smc5-33 cells exhibit hypersensitivity to several DNA-damaging agents despite induction of the DNA damage checkpoint .
	manualset3
255968	4	423953	15	NULL	NULL	NULL	NULL	hypersensitivity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the permissive temperature , smc5-31 but not smc5-33 cells exhibit hypersensitivity to several DNA-damaging agents despite induction of the DNA damage checkpoint .
	manualset3
255969	5	423953	15	NULL	NULL	NULL	NULL	DNA-damaging agents	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the permissive temperature , smc5-31 but not smc5-33 cells exhibit hypersensitivity to several DNA-damaging agents despite induction of the DNA damage checkpoint .
	manualset3
255970	6	423953	15	NULL	NULL	NULL	NULL	induction	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the permissive temperature , smc5-31 but not smc5-33 cells exhibit hypersensitivity to several DNA-damaging agents despite induction of the DNA damage checkpoint .
	manualset3
255971	7	423953	15	NULL	NULL	NULL	NULL	DNA damage checkpoint	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the permissive temperature , smc5-31 but not smc5-33 cells exhibit hypersensitivity to several DNA-damaging agents despite induction of the DNA damage checkpoint .
	manualset3
255972	1	423954	15	NULL	NULL	NULL	NULL	present time	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the present time , when physical health is constantly improving , the most pressing problems are those related to lifestyle and mental health which depend for a large part on social factors .
	manualset3
255973	2	423954	15	NULL	NULL	NULL	NULL	physical health 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the present time , when physical health is constantly improving , the most pressing problems are those related to lifestyle and mental health which depend for a large part on social factors .
	manualset3
255974	3	423954	15	NULL	NULL	NULL	NULL	improving	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the present time , when physical health is constantly improving , the most pressing problems are those related to lifestyle and mental health which depend for a large part on social factors .
	manualset3
255975	4	423954	15	NULL	NULL	NULL	NULL	problems	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the present time , when physical health is constantly improving , the most pressing problems are those related to lifestyle and mental health which depend for a large part on social factors .
	manualset3
255976	5	423954	15	NULL	NULL	NULL	NULL	lifestyle	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the present time , when physical health is constantly improving , the most pressing problems are those related to lifestyle and mental health which depend for a large part on social factors .
	manualset3
255977	6	423954	15	NULL	NULL	NULL	NULL	mental health	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the present time , when physical health is constantly improving , the most pressing problems are those related to lifestyle and mental health which depend for a large part on social factors .
	manualset3
255978	7	423954	15	NULL	NULL	NULL	NULL	part 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the present time , when physical health is constantly improving , the most pressing problems are those related to lifestyle and mental health which depend for a large part on social factors .
	manualset3
255979	8	423954	15	NULL	NULL	NULL	NULL	social factors	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the present time , when physical health is constantly improving , the most pressing problems are those related to lifestyle and mental health which depend for a large part on social factors .
	manualset3
255980	1	423955	15	NULL	NULL	NULL	NULL	same time	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the same time , we found regions that correspond to 16S rRNA fragments distant from the binding sites of the respective homologous prokaryotic proteins .
	manualset3
255981	2	423955	15	NULL	NULL	NULL	NULL	regions	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the same time , we found regions that correspond to 16S rRNA fragments distant from the binding sites of the respective homologous prokaryotic proteins .
	manualset3
255982	3	423955	15	NULL	NULL	NULL	NULL	16S rRNA fragments 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the same time , we found regions that correspond to 16S rRNA fragments distant from the binding sites of the respective homologous prokaryotic proteins .
	manualset3
255983	4	423955	15	NULL	NULL	NULL	NULL	binding sites	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the same time , we found regions that correspond to 16S rRNA fragments distant from the binding sites of the respective homologous prokaryotic proteins .
	manualset3
255984	5	423955	15	NULL	NULL	NULL	NULL	respective homologous prokaryotic proteins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the same time , we found regions that correspond to 16S rRNA fragments distant from the binding sites of the respective homologous prokaryotic proteins .
	manualset3
255985	1	423956	15	NULL	NULL	NULL	NULL	same time	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the same time application of therapy is suggested right after the diagnosis is set , even though the patient may be in the early clinical stadium of the disease , as well as the decision about aggressive treatment .
	manualset3
255986	2	423956	15	NULL	NULL	NULL	NULL	application of therapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the same time application of therapy is suggested right after the diagnosis is set , even though the patient may be in the early clinical stadium of the disease , as well as the decision about aggressive treatment .
	manualset3
255987	3	423956	15	NULL	NULL	NULL	NULL	diagnosis	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the same time application of therapy is suggested right after the diagnosis is set , even though the patient may be in the early clinical stadium of the disease , as well as the decision about aggressive treatment .
	manualset3
255988	4	423956	15	NULL	NULL	NULL	NULL	patient 	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the same time application of therapy is suggested right after the diagnosis is set , even though the patient may be in the early clinical stadium of the disease , as well as the decision about aggressive treatment .
	manualset3
255989	5	423956	15	NULL	NULL	NULL	NULL	early clinical stadium of the disease	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the same time application of therapy is suggested right after the diagnosis is set , even though the patient may be in the early clinical stadium of the disease , as well as the decision about aggressive treatment .
	manualset3
255990	6	423956	15	NULL	NULL	NULL	NULL	decision	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the same time application of therapy is suggested right after the diagnosis is set , even though the patient may be in the early clinical stadium of the disease , as well as the decision about aggressive treatment .
	manualset3
255991	7	423956	15	NULL	NULL	NULL	NULL	aggressive treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the same time application of therapy is suggested right after the diagnosis is set , even though the patient may be in the early clinical stadium of the disease , as well as the decision about aggressive treatment .
	manualset3
255992	1	423957	15	NULL	NULL	NULL	NULL	scene	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the scene were numerous bottles of methadone , with the chronic dosage of 240 mg 3 times a day .
	manualset3
255993	2	423957	15	NULL	NULL	NULL	NULL	numerous bottles 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the scene were numerous bottles of methadone , with the chronic dosage of 240 mg 3 times a day .
	manualset3
255994	3	423957	15	NULL	NULL	NULL	NULL	methadone	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the scene were numerous bottles of methadone , with the chronic dosage of 240 mg 3 times a day .
	manualset3
255995	4	423957	15	NULL	NULL	NULL	NULL	chronic dosage of 240 mg	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the scene were numerous bottles of methadone , with the chronic dosage of 240 mg 3 times a day .
	manualset3
255996	5	423957	15	NULL	NULL	NULL	NULL	3 times a day	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the scene were numerous bottles of methadone , with the chronic dosage of 240 mg 3 times a day .
	manualset3
255997	1	423958	15	NULL	NULL	NULL	NULL	site of the carcinoma 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the site of the carcinoma , 36 ( 54 % ) had hypofunction , associated with a palpable abnormality in all but one patient ; 16 ( 24 % ) had an abnormality on palpation but not on scanning ; 11 ( 16 % ) had both a normal clinical examination and a normal scan , associated with a benign abnormality in another part of the thyroid ; and four ( 6 % ) had a patchy uptake .
	manualset3
255998	2	423958	15	NULL	NULL	NULL	NULL	36 ( 54 % )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the site of the carcinoma , 36 ( 54 % ) had hypofunction , associated with a palpable abnormality in all but one patient ; 16 ( 24 % ) had an abnormality on palpation but not on scanning ; 11 ( 16 % ) had both a normal clinical examination and a normal scan , associated with a benign abnormality in another part of the thyroid ; and four ( 6 % ) had a patchy uptake .
	manualset3
255999	3	423958	15	NULL	NULL	NULL	NULL	hypofunction	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the site of the carcinoma , 36 ( 54 % ) had hypofunction , associated with a palpable abnormality in all but one patient ; 16 ( 24 % ) had an abnormality on palpation but not on scanning ; 11 ( 16 % ) had both a normal clinical examination and a normal scan , associated with a benign abnormality in another part of the thyroid ; and four ( 6 % ) had a patchy uptake .
	manualset3
256000	4	423958	15	NULL	NULL	NULL	NULL	palpable abnormality	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the site of the carcinoma , 36 ( 54 % ) had hypofunction , associated with a palpable abnormality in all but one patient ; 16 ( 24 % ) had an abnormality on palpation but not on scanning ; 11 ( 16 % ) had both a normal clinical examination and a normal scan , associated with a benign abnormality in another part of the thyroid ; and four ( 6 % ) had a patchy uptake .
	manualset3
256001	5	423958	15	NULL	NULL	NULL	NULL	one patient 	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the site of the carcinoma , 36 ( 54 % ) had hypofunction , associated with a palpable abnormality in all but one patient ; 16 ( 24 % ) had an abnormality on palpation but not on scanning ; 11 ( 16 % ) had both a normal clinical examination and a normal scan , associated with a benign abnormality in another part of the thyroid ; and four ( 6 % ) had a patchy uptake .
	manualset3
256002	6	423958	15	NULL	NULL	NULL	NULL	16 ( 24 % )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the site of the carcinoma , 36 ( 54 % ) had hypofunction , associated with a palpable abnormality in all but one patient ; 16 ( 24 % ) had an abnormality on palpation but not on scanning ; 11 ( 16 % ) had both a normal clinical examination and a normal scan , associated with a benign abnormality in another part of the thyroid ; and four ( 6 % ) had a patchy uptake .
	manualset3
256003	7	423958	15	NULL	NULL	NULL	NULL	abnormality on palpation 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the site of the carcinoma , 36 ( 54 % ) had hypofunction , associated with a palpable abnormality in all but one patient ; 16 ( 24 % ) had an abnormality on palpation but not on scanning ; 11 ( 16 % ) had both a normal clinical examination and a normal scan , associated with a benign abnormality in another part of the thyroid ; and four ( 6 % ) had a patchy uptake .
	manualset3
256004	8	423958	15	NULL	NULL	NULL	NULL	scanning	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the site of the carcinoma , 36 ( 54 % ) had hypofunction , associated with a palpable abnormality in all but one patient ; 16 ( 24 % ) had an abnormality on palpation but not on scanning ; 11 ( 16 % ) had both a normal clinical examination and a normal scan , associated with a benign abnormality in another part of the thyroid ; and four ( 6 % ) had a patchy uptake .
	manualset3
256005	9	423958	15	NULL	NULL	NULL	NULL	11 ( 16 % ) 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the site of the carcinoma , 36 ( 54 % ) had hypofunction , associated with a palpable abnormality in all but one patient ; 16 ( 24 % ) had an abnormality on palpation but not on scanning ; 11 ( 16 % ) had both a normal clinical examination and a normal scan , associated with a benign abnormality in another part of the thyroid ; and four ( 6 % ) had a patchy uptake .
	manualset3
256006	10	423958	15	NULL	NULL	NULL	NULL	normal clinical examination	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the site of the carcinoma , 36 ( 54 % ) had hypofunction , associated with a palpable abnormality in all but one patient ; 16 ( 24 % ) had an abnormality on palpation but not on scanning ; 11 ( 16 % ) had both a normal clinical examination and a normal scan , associated with a benign abnormality in another part of the thyroid ; and four ( 6 % ) had a patchy uptake .
	manualset3
256007	11	423958	15	NULL	NULL	NULL	NULL	normal scan	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the site of the carcinoma , 36 ( 54 % ) had hypofunction , associated with a palpable abnormality in all but one patient ; 16 ( 24 % ) had an abnormality on palpation but not on scanning ; 11 ( 16 % ) had both a normal clinical examination and a normal scan , associated with a benign abnormality in another part of the thyroid ; and four ( 6 % ) had a patchy uptake .
	manualset3
256008	12	423958	15	NULL	NULL	NULL	NULL	benign abnormality 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the site of the carcinoma , 36 ( 54 % ) had hypofunction , associated with a palpable abnormality in all but one patient ; 16 ( 24 % ) had an abnormality on palpation but not on scanning ; 11 ( 16 % ) had both a normal clinical examination and a normal scan , associated with a benign abnormality in another part of the thyroid ; and four ( 6 % ) had a patchy uptake .
	manualset3
256009	13	423958	15	NULL	NULL	NULL	NULL	part of the thyroid	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the site of the carcinoma , 36 ( 54 % ) had hypofunction , associated with a palpable abnormality in all but one patient ; 16 ( 24 % ) had an abnormality on palpation but not on scanning ; 11 ( 16 % ) had both a normal clinical examination and a normal scan , associated with a benign abnormality in another part of the thyroid ; and four ( 6 % ) had a patchy uptake .
	manualset3
256010	14	423958	15	NULL	NULL	NULL	NULL	four ( 6 % ) 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the site of the carcinoma , 36 ( 54 % ) had hypofunction , associated with a palpable abnormality in all but one patient ; 16 ( 24 % ) had an abnormality on palpation but not on scanning ; 11 ( 16 % ) had both a normal clinical examination and a normal scan , associated with a benign abnormality in another part of the thyroid ; and four ( 6 % ) had a patchy uptake .
	manualset3
256011	15	423958	15	NULL	NULL	NULL	NULL	patchy uptake	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the site of the carcinoma , 36 ( 54 % ) had hypofunction , associated with a palpable abnormality in all but one patient ; 16 ( 24 % ) had an abnormality on palpation but not on scanning ; 11 ( 16 % ) had both a normal clinical examination and a normal scan , associated with a benign abnormality in another part of the thyroid ; and four ( 6 % ) had a patchy uptake .
	manualset3
256012	1	423959	15	NULL	NULL	NULL	NULL	stable period	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the stable period , low-dose aspirin inhibited platelet aggregation induced by ADP , collagen , or arachidonic acid , and suppressed the increase in intracellular Ca2 + concentration ( ( Ca2 + ) i ) induced by thrombin significantly .
	manualset3
256013	2	423959	15	NULL	NULL	NULL	NULL	low-dose	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the stable period , low-dose aspirin inhibited platelet aggregation induced by ADP , collagen , or arachidonic acid , and suppressed the increase in intracellular Ca2 + concentration ( ( Ca2 + ) i ) induced by thrombin significantly .
	manualset3
256014	3	423959	15	NULL	NULL	NULL	NULL	aspirin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the stable period , low-dose aspirin inhibited platelet aggregation induced by ADP , collagen , or arachidonic acid , and suppressed the increase in intracellular Ca2 + concentration ( ( Ca2 + ) i ) induced by thrombin significantly .
	manualset3
256015	4	423959	15	NULL	NULL	NULL	NULL	platelet aggregation 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the stable period , low-dose aspirin inhibited platelet aggregation induced by ADP , collagen , or arachidonic acid , and suppressed the increase in intracellular Ca2 + concentration ( ( Ca2 + ) i ) induced by thrombin significantly .
	manualset3
256016	5	423959	15	NULL	NULL	NULL	NULL	ADP	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the stable period , low-dose aspirin inhibited platelet aggregation induced by ADP , collagen , or arachidonic acid , and suppressed the increase in intracellular Ca2 + concentration ( ( Ca2 + ) i ) induced by thrombin significantly .
	manualset3
256017	6	423959	15	NULL	NULL	NULL	NULL	collagen	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the stable period , low-dose aspirin inhibited platelet aggregation induced by ADP , collagen , or arachidonic acid , and suppressed the increase in intracellular Ca2 + concentration ( ( Ca2 + ) i ) induced by thrombin significantly .
	manualset3
256018	7	423959	15	NULL	NULL	NULL	NULL	arachidonic acid	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the stable period , low-dose aspirin inhibited platelet aggregation induced by ADP , collagen , or arachidonic acid , and suppressed the increase in intracellular Ca2 + concentration ( ( Ca2 + ) i ) induced by thrombin significantly .
	manualset3
256019	8	423959	15	NULL	NULL	NULL	NULL	increase	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the stable period , low-dose aspirin inhibited platelet aggregation induced by ADP , collagen , or arachidonic acid , and suppressed the increase in intracellular Ca2 + concentration ( ( Ca2 + ) i ) induced by thrombin significantly .
	manualset3
256020	9	423959	15	NULL	NULL	NULL	NULL	intracellular Ca2 + concentration 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the stable period , low-dose aspirin inhibited platelet aggregation induced by ADP , collagen , or arachidonic acid , and suppressed the increase in intracellular Ca2 + concentration ( ( Ca2 + ) i ) induced by thrombin significantly .
	manualset3
256021	11	423959	15	NULL	NULL	NULL	NULL	thrombin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the stable period , low-dose aspirin inhibited platelet aggregation induced by ADP , collagen , or arachidonic acid , and suppressed the increase in intracellular Ca2 + concentration ( ( Ca2 + ) i ) induced by thrombin significantly .
	manualset3
256022	10	423959	15	NULL	NULL	NULL	NULL	( ( Ca2 + ) i )	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the stable period , low-dose aspirin inhibited platelet aggregation induced by ADP , collagen , or arachidonic acid , and suppressed the increase in intracellular Ca2 + concentration ( ( Ca2 + ) i ) induced by thrombin significantly .
	manualset3
256023	1	423960	15	NULL	NULL	NULL	NULL	stationary phase 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the stationary phase of cell growth , the NO3 - and NH4 + disappeared entirely from the medium .
	manualset3
256024	2	423960	15	NULL	NULL	NULL	NULL	cell growth	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the stationary phase of cell growth , the NO3 - and NH4 + disappeared entirely from the medium .
	manualset3
256025	3	423960	15	NULL	NULL	NULL	NULL	NO3 -	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the stationary phase of cell growth , the NO3 - and NH4 + disappeared entirely from the medium .
	manualset3
256026	4	423960	15	NULL	NULL	NULL	NULL	NH4 +	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the stationary phase of cell growth , the NO3 - and NH4 + disappeared entirely from the medium .
	manualset3
256027	5	423960	15	NULL	NULL	NULL	NULL	 medium	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the stationary phase of cell growth , the NO3 - and NH4 + disappeared entirely from the medium .
	manualset3
256028	1	423961	15	NULL	NULL	NULL	NULL	study 's completion	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the study 's completion , marrow cellularities and peripheral blood counts of the remaining young and elderly dogs were equivalent .
	manualset3
256029	2	423961	15	NULL	NULL	NULL	NULL	marrow cellularities	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the study 's completion , marrow cellularities and peripheral blood counts of the remaining young and elderly dogs were equivalent .
	manualset3
256030	3	423961	15	NULL	NULL	NULL	NULL	peripheral blood counts 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the study 's completion , marrow cellularities and peripheral blood counts of the remaining young and elderly dogs were equivalent .
	manualset3
256031	4	423961	15	NULL	NULL	NULL	NULL	young dogs	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the study 's completion , marrow cellularities and peripheral blood counts of the remaining young and elderly dogs were equivalent .
	manualset3
259682	5	423961	15	NULL	NULL	NULL	NULL	elderly dogs 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the study 's completion , marrow cellularities and peripheral blood counts of the remaining young and elderly dogs were equivalent .
	manualset3
256032	1	423962	15	NULL	NULL	NULL	NULL	time 	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the time of embolization active contrast extravasation was seen in 36 of 57 patients , while in the remaining 21 patients embolization was based on endoscopic findings .
	manualset3
256033	2	423962	15	NULL	NULL	NULL	NULL	embolization	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the time of embolization active contrast extravasation was seen in 36 of 57 patients , while in the remaining 21 patients embolization was based on endoscopic findings .
	manualset3
256034	3	423962	15	NULL	NULL	NULL	NULL	active contrast extravasation 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the time of embolization active contrast extravasation was seen in 36 of 57 patients , while in the remaining 21 patients embolization was based on endoscopic findings .
	manualset3
256035	4	423962	15	NULL	NULL	NULL	NULL	36 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the time of embolization active contrast extravasation was seen in 36 of 57 patients , while in the remaining 21 patients embolization was based on endoscopic findings .
	manualset3
256036	5	423962	15	NULL	NULL	NULL	NULL	57 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the time of embolization active contrast extravasation was seen in 36 of 57 patients , while in the remaining 21 patients embolization was based on endoscopic findings .
	manualset3
256037	6	423962	15	NULL	NULL	NULL	NULL	21 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the time of embolization active contrast extravasation was seen in 36 of 57 patients , while in the remaining 21 patients embolization was based on endoscopic findings .
	manualset3
256038	7	423962	15	NULL	NULL	NULL	NULL	embolization	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the time of embolization active contrast extravasation was seen in 36 of 57 patients , while in the remaining 21 patients embolization was based on endoscopic findings .
	manualset3
256039	8	423962	15	NULL	NULL	NULL	NULL	endoscopic findings 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the time of embolization active contrast extravasation was seen in 36 of 57 patients , while in the remaining 21 patients embolization was based on endoscopic findings .
	manualset3
256040	1	423963	15	NULL	NULL	NULL	NULL	time 	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the time of laparotomy , the placenta was removed completely with good maternal outcome .
	manualset3
256041	2	423963	15	NULL	NULL	NULL	NULL	laparotomy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the time of laparotomy , the placenta was removed completely with good maternal outcome .
	manualset3
256042	3	423963	15	NULL	NULL	NULL	NULL	placenta	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the time of laparotomy , the placenta was removed completely with good maternal outcome .
	manualset3
256043	4	423963	15	NULL	NULL	NULL	NULL	good maternal outcome	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the time of laparotomy , the placenta was removed completely with good maternal outcome .
	manualset3
256044	1	423964	15	NULL	NULL	NULL	NULL	time 	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the time of maximum depression of the blood cell counts , the hematocrit value was 21 % ; the WBC count , 1 , 000 / cu mm ; and the platelet count , 27 , 000 / cu mm .
	manualset3
256045	2	423964	15	NULL	NULL	NULL	NULL	depression of the blood cell counts	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the time of maximum depression of the blood cell counts , the hematocrit value was 21 % ; the WBC count , 1 , 000 / cu mm ; and the platelet count , 27 , 000 / cu mm .
	manualset3
256046	3	423964	15	NULL	NULL	NULL	NULL	hematocrit value	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the time of maximum depression of the blood cell counts , the hematocrit value was 21 % ; the WBC count , 1 , 000 / cu mm ; and the platelet count , 27 , 000 / cu mm .
	manualset3
256047	4	423964	15	NULL	NULL	NULL	NULL	21 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the time of maximum depression of the blood cell counts , the hematocrit value was 21 % ; the WBC count , 1 , 000 / cu mm ; and the platelet count , 27 , 000 / cu mm .
	manualset3
256048	5	423964	15	NULL	NULL	NULL	NULL	WBC count	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the time of maximum depression of the blood cell counts , the hematocrit value was 21 % ; the WBC count , 1 , 000 / cu mm ; and the platelet count , 27 , 000 / cu mm .
	manualset3
256049	6	423964	15	NULL	NULL	NULL	NULL	1 , 000 / cu mm	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the time of maximum depression of the blood cell counts , the hematocrit value was 21 % ; the WBC count , 1 , 000 / cu mm ; and the platelet count , 27 , 000 / cu mm .
	manualset3
256050	7	423964	15	NULL	NULL	NULL	NULL	platelet count	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the time of maximum depression of the blood cell counts , the hematocrit value was 21 % ; the WBC count , 1 , 000 / cu mm ; and the platelet count , 27 , 000 / cu mm .
	manualset3
256051	8	423964	15	NULL	NULL	NULL	NULL	27 , 000 / cu mm	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the time of maximum depression of the blood cell counts , the hematocrit value was 21 % ; the WBC count , 1 , 000 / cu mm ; and the platelet count , 27 , 000 / cu mm .
	manualset3
256052	1	423965	15	NULL	NULL	NULL	NULL	two ends	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the two ends of vertical interface , two salt bridges are formed between pairs of Lys41-Asp233 and Lys68-Glu229 .
	manualset3
256053	2	423965	15	NULL	NULL	NULL	NULL	vertical interface 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the two ends of vertical interface , two salt bridges are formed between pairs of Lys41-Asp233 and Lys68-Glu229 .
	manualset3
256054	3	423965	15	NULL	NULL	NULL	NULL	two salt bridges	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the two ends of vertical interface , two salt bridges are formed between pairs of Lys41-Asp233 and Lys68-Glu229 .
	manualset3
256055	4	423965	15	NULL	NULL	NULL	NULL	pairs	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the two ends of vertical interface , two salt bridges are formed between pairs of Lys41-Asp233 and Lys68-Glu229 .
	manualset3
256056	5	423965	15	NULL	NULL	NULL	NULL	Lys41-Asp233	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the two ends of vertical interface , two salt bridges are formed between pairs of Lys41-Asp233 and Lys68-Glu229 .
	manualset3
256057	6	423965	15	NULL	NULL	NULL	NULL	Lys68-Glu229	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the two ends of vertical interface , two salt bridges are formed between pairs of Lys41-Asp233 and Lys68-Glu229 .
	manualset3
256397	1	423966	15	NULL	NULL	NULL	NULL	ultrastructural level	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the ultrastructural level , best visualized with the PA-CrA-silver technique , granule discharge was observed , as was an overall increase in size of the granules .
	manualset3
256398	2	423966	15	NULL	NULL	NULL	NULL	PA-CrA-silver technique	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the ultrastructural level , best visualized with the PA-CrA-silver technique , granule discharge was observed , as was an overall increase in size of the granules .
	manualset3
256399	3	423966	15	NULL	NULL	NULL	NULL	granule discharge	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the ultrastructural level , best visualized with the PA-CrA-silver technique , granule discharge was observed , as was an overall increase in size of the granules .
	manualset3
256400	4	423966	15	NULL	NULL	NULL	NULL	increase	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the ultrastructural level , best visualized with the PA-CrA-silver technique , granule discharge was observed , as was an overall increase in size of the granules .
	manualset3
256401	5	423966	15	NULL	NULL	NULL	NULL	size	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the ultrastructural level , best visualized with the PA-CrA-silver technique , granule discharge was observed , as was an overall increase in size of the granules .
	manualset3
256402	6	423966	15	NULL	NULL	NULL	NULL	granules	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the ultrastructural level , best visualized with the PA-CrA-silver technique , granule discharge was observed , as was an overall increase in size of the granules .
	manualset3
256403	1	423967	15	NULL	NULL	NULL	NULL	ultrastructural level	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the ultrastructural level , the amount of glycogen in trophoblast layer II was elevated in cadmium exposed rats , but other electron microscopic features ( amount and localization of lipid , degenerative vesicles , thickness and general appearance of the trophoblastic and endothelial layers and thickening or multiplication of the basal lamina ) were not changed .
	manualset3
256404	2	423967	15	NULL	NULL	NULL	NULL	amount	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the ultrastructural level , the amount of glycogen in trophoblast layer II was elevated in cadmium exposed rats , but other electron microscopic features ( amount and localization of lipid , degenerative vesicles , thickness and general appearance of the trophoblastic and endothelial layers and thickening or multiplication of the basal lamina ) were not changed .
	manualset3
256406	3	423967	15	NULL	NULL	NULL	NULL	glycogen 	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the ultrastructural level , the amount of glycogen in trophoblast layer II was elevated in cadmium exposed rats , but other electron microscopic features ( amount and localization of lipid , degenerative vesicles , thickness and general appearance of the trophoblastic and endothelial layers and thickening or multiplication of the basal lamina ) were not changed .
	manualset3
256407	4	423967	15	NULL	NULL	NULL	NULL	trophoblast layer II	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the ultrastructural level , the amount of glycogen in trophoblast layer II was elevated in cadmium exposed rats , but other electron microscopic features ( amount and localization of lipid , degenerative vesicles , thickness and general appearance of the trophoblastic and endothelial layers and thickening or multiplication of the basal lamina ) were not changed .
	manualset3
256410	5	423967	15	NULL	NULL	NULL	NULL	cadmium	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the ultrastructural level , the amount of glycogen in trophoblast layer II was elevated in cadmium exposed rats , but other electron microscopic features ( amount and localization of lipid , degenerative vesicles , thickness and general appearance of the trophoblastic and endothelial layers and thickening or multiplication of the basal lamina ) were not changed .
	manualset3
256412	6	423967	15	NULL	NULL	NULL	NULL	rats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the ultrastructural level , the amount of glycogen in trophoblast layer II was elevated in cadmium exposed rats , but other electron microscopic features ( amount and localization of lipid , degenerative vesicles , thickness and general appearance of the trophoblastic and endothelial layers and thickening or multiplication of the basal lamina ) were not changed .
	manualset3
256414	7	423967	15	NULL	NULL	NULL	NULL	electron microscopic features	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the ultrastructural level , the amount of glycogen in trophoblast layer II was elevated in cadmium exposed rats , but other electron microscopic features ( amount and localization of lipid , degenerative vesicles , thickness and general appearance of the trophoblastic and endothelial layers and thickening or multiplication of the basal lamina ) were not changed .
	manualset3
256415	8	423967	15	NULL	NULL	NULL	NULL	amount of lipid	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the ultrastructural level , the amount of glycogen in trophoblast layer II was elevated in cadmium exposed rats , but other electron microscopic features ( amount and localization of lipid , degenerative vesicles , thickness and general appearance of the trophoblastic and endothelial layers and thickening or multiplication of the basal lamina ) were not changed .
	manualset3
256416	9	423967	15	NULL	NULL	NULL	NULL	localization of lipid 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the ultrastructural level , the amount of glycogen in trophoblast layer II was elevated in cadmium exposed rats , but other electron microscopic features ( amount and localization of lipid , degenerative vesicles , thickness and general appearance of the trophoblastic and endothelial layers and thickening or multiplication of the basal lamina ) were not changed .
	manualset3
256417	10	423967	15	NULL	NULL	NULL	NULL	vesicles	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the ultrastructural level , the amount of glycogen in trophoblast layer II was elevated in cadmium exposed rats , but other electron microscopic features ( amount and localization of lipid , degenerative vesicles , thickness and general appearance of the trophoblastic and endothelial layers and thickening or multiplication of the basal lamina ) were not changed .
	manualset3
256418	11	423967	15	NULL	NULL	NULL	NULL	thickness	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the ultrastructural level , the amount of glycogen in trophoblast layer II was elevated in cadmium exposed rats , but other electron microscopic features ( amount and localization of lipid , degenerative vesicles , thickness and general appearance of the trophoblastic and endothelial layers and thickening or multiplication of the basal lamina ) were not changed .
	manualset3
256419	12	423967	15	NULL	NULL	NULL	NULL	appearance	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the ultrastructural level , the amount of glycogen in trophoblast layer II was elevated in cadmium exposed rats , but other electron microscopic features ( amount and localization of lipid , degenerative vesicles , thickness and general appearance of the trophoblastic and endothelial layers and thickening or multiplication of the basal lamina ) were not changed .
	manualset3
256420	13	423967	15	NULL	NULL	NULL	NULL	trophoblastic layers	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the ultrastructural level , the amount of glycogen in trophoblast layer II was elevated in cadmium exposed rats , but other electron microscopic features ( amount and localization of lipid , degenerative vesicles , thickness and general appearance of the trophoblastic and endothelial layers and thickening or multiplication of the basal lamina ) were not changed .
	manualset3
256421	14	423967	15	NULL	NULL	NULL	NULL	endothelial layers	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the ultrastructural level , the amount of glycogen in trophoblast layer II was elevated in cadmium exposed rats , but other electron microscopic features ( amount and localization of lipid , degenerative vesicles , thickness and general appearance of the trophoblastic and endothelial layers and thickening or multiplication of the basal lamina ) were not changed .
	manualset3
256422	15	423967	15	NULL	NULL	NULL	NULL	thickening of the basal lamina	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the ultrastructural level , the amount of glycogen in trophoblast layer II was elevated in cadmium exposed rats , but other electron microscopic features ( amount and localization of lipid , degenerative vesicles , thickness and general appearance of the trophoblastic and endothelial layers and thickening or multiplication of the basal lamina ) were not changed .
	manualset3
256423	16	423967	15	NULL	NULL	NULL	NULL	multiplication of the basal lamina	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the ultrastructural level , the amount of glycogen in trophoblast layer II was elevated in cadmium exposed rats , but other electron microscopic features ( amount and localization of lipid , degenerative vesicles , thickness and general appearance of the trophoblastic and endothelial layers and thickening or multiplication of the basal lamina ) were not changed .
	manualset3
256425	1	423968	15	NULL	NULL	NULL	NULL	yellow gene	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the yellow gene , transvection is the basis for several examples of intragenic complementation involving the enhancers of one allele acting in trans on the promoter of a paired second allele .
	manualset3
256426	2	423968	15	NULL	NULL	NULL	NULL	transvection	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the yellow gene , transvection is the basis for several examples of intragenic complementation involving the enhancers of one allele acting in trans on the promoter of a paired second allele .
	manualset3
256427	3	423968	15	NULL	NULL	NULL	NULL	 basis	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the yellow gene , transvection is the basis for several examples of intragenic complementation involving the enhancers of one allele acting in trans on the promoter of a paired second allele .
	manualset3
256428	4	423968	15	NULL	NULL	NULL	NULL	examples 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the yellow gene , transvection is the basis for several examples of intragenic complementation involving the enhancers of one allele acting in trans on the promoter of a paired second allele .
	manualset3
256429	5	423968	15	NULL	NULL	NULL	NULL	intragenic complementation 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the yellow gene , transvection is the basis for several examples of intragenic complementation involving the enhancers of one allele acting in trans on the promoter of a paired second allele .
	manualset3
256430	6	423968	15	NULL	NULL	NULL	NULL	enhancers 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the yellow gene , transvection is the basis for several examples of intragenic complementation involving the enhancers of one allele acting in trans on the promoter of a paired second allele .
	manualset3
256431	7	423968	15	NULL	NULL	NULL	NULL	allele 	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the yellow gene , transvection is the basis for several examples of intragenic complementation involving the enhancers of one allele acting in trans on the promoter of a paired second allele .
	manualset3
256432	8	423968	15	NULL	NULL	NULL	NULL	trans	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the yellow gene , transvection is the basis for several examples of intragenic complementation involving the enhancers of one allele acting in trans on the promoter of a paired second allele .
	manualset3
256433	9	423968	15	NULL	NULL	NULL	NULL	promoter 	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the yellow gene , transvection is the basis for several examples of intragenic complementation involving the enhancers of one allele acting in trans on the promoter of a paired second allele .
	manualset3
256434	10	423968	15	NULL	NULL	NULL	NULL	allele	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At the yellow gene , transvection is the basis for several examples of intragenic complementation involving the enhancers of one allele acting in trans on the promoter of a paired second allele .
	manualset3
256437	1	423969	15	NULL	NULL	NULL	NULL	time	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At this time , although a smaller intensity of renal papillary necrosis was observed with the amino acid mixture pretreatment , N-acetyl-L-cysteine pretreated rats showed no papillary necrosis .
	manualset3
256439	2	423969	15	NULL	NULL	NULL	NULL	intensity 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At this time , although a smaller intensity of renal papillary necrosis was observed with the amino acid mixture pretreatment , N-acetyl-L-cysteine pretreated rats showed no papillary necrosis .
	manualset3
256440	3	423969	15	NULL	NULL	NULL	NULL	renal papillary necrosis 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At this time , although a smaller intensity of renal papillary necrosis was observed with the amino acid mixture pretreatment , N-acetyl-L-cysteine pretreated rats showed no papillary necrosis .
	manualset3
256442	4	423969	15	NULL	NULL	NULL	NULL	amino acid mixture pretreatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At this time , although a smaller intensity of renal papillary necrosis was observed with the amino acid mixture pretreatment , N-acetyl-L-cysteine pretreated rats showed no papillary necrosis .
	manualset3
256444	5	423969	15	NULL	NULL	NULL	NULL	N-acetyl-L-cysteine	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At this time , although a smaller intensity of renal papillary necrosis was observed with the amino acid mixture pretreatment , N-acetyl-L-cysteine pretreated rats showed no papillary necrosis .
	manualset3
256445	6	423969	15	NULL	NULL	NULL	NULL	rats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At this time , although a smaller intensity of renal papillary necrosis was observed with the amino acid mixture pretreatment , N-acetyl-L-cysteine pretreated rats showed no papillary necrosis .
	manualset3
256446	7	423969	15	NULL	NULL	NULL	NULL	papillary necrosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At this time , although a smaller intensity of renal papillary necrosis was observed with the amino acid mixture pretreatment , N-acetyl-L-cysteine pretreated rats showed no papillary necrosis .
	manualset3
256451	1	423970	15	NULL	NULL	NULL	NULL	 time	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At this time , the rabbits became hypotensive , O2 delivery to the brain decreased dramatically and the CSER could not be elicited .
	manualset3
256452	2	423970	15	NULL	NULL	NULL	NULL	rabbits	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At this time , the rabbits became hypotensive , O2 delivery to the brain decreased dramatically and the CSER could not be elicited .
	manualset3
256455	3	423970	15	NULL	NULL	NULL	NULL	hypotensive	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At this time , the rabbits became hypotensive , O2 delivery to the brain decreased dramatically and the CSER could not be elicited .
	manualset3
256457	4	423970	15	NULL	NULL	NULL	NULL	O2 delivery	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At this time , the rabbits became hypotensive , O2 delivery to the brain decreased dramatically and the CSER could not be elicited .
	manualset3
256458	5	423970	15	NULL	NULL	NULL	NULL	brain	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At this time , the rabbits became hypotensive , O2 delivery to the brain decreased dramatically and the CSER could not be elicited .
	manualset3
256460	6	423970	15	NULL	NULL	NULL	NULL	CSER	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At this time , the rabbits became hypotensive , O2 delivery to the brain decreased dramatically and the CSER could not be elicited .
	manualset3
256462	1	423971	15	NULL	NULL	NULL	NULL	three months posttreatment	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At three months posttreatment , the inpatient group had a statistically significant higher rate of total abstinence than the day-treatment group , but the difference at six months was not statistically significant .
	manualset3
256463	2	423971	15	NULL	NULL	NULL	NULL	inpatient group	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At three months posttreatment , the inpatient group had a statistically significant higher rate of total abstinence than the day-treatment group , but the difference at six months was not statistically significant .
	manualset3
256467	3	423971	15	NULL	NULL	NULL	NULL	rate	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At three months posttreatment , the inpatient group had a statistically significant higher rate of total abstinence than the day-treatment group , but the difference at six months was not statistically significant .
	manualset3
256471	4	423971	15	NULL	NULL	NULL	NULL	abstinence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At three months posttreatment , the inpatient group had a statistically significant higher rate of total abstinence than the day-treatment group , but the difference at six months was not statistically significant .
	manualset3
256472	5	423971	15	NULL	NULL	NULL	NULL	day-treatment group	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At three months posttreatment , the inpatient group had a statistically significant higher rate of total abstinence than the day-treatment group , but the difference at six months was not statistically significant .
	manualset3
256473	6	423971	15	NULL	NULL	NULL	NULL	difference 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At three months posttreatment , the inpatient group had a statistically significant higher rate of total abstinence than the day-treatment group , but the difference at six months was not statistically significant .
	manualset3
256474	7	423971	15	NULL	NULL	NULL	NULL	 six months	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At three months posttreatment , the inpatient group had a statistically significant higher rate of total abstinence than the day-treatment group , but the difference at six months was not statistically significant .
	manualset3
256477	1	423972	15	NULL	NULL	NULL	NULL	week twelve	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At week twelve , 38 % of the DMAS users and 14 % of the control subjects had an undetectable plasma HIV RNA load ( P = .014 ) , and at week 24 , the plasma HIV RNA load was undetectable for 34 % of the DMAS users and 38 % of the control subjects ( P = .49 ) .
	manualset3
256478	2	423972	15	NULL	NULL	NULL	NULL	38 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At week twelve , 38 % of the DMAS users and 14 % of the control subjects had an undetectable plasma HIV RNA load ( P = .014 ) , and at week 24 , the plasma HIV RNA load was undetectable for 34 % of the DMAS users and 38 % of the control subjects ( P = .49 ) .
	manualset3
256480	3	423972	15	NULL	NULL	NULL	NULL	DMAS users	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At week twelve , 38 % of the DMAS users and 14 % of the control subjects had an undetectable plasma HIV RNA load ( P = .014 ) , and at week 24 , the plasma HIV RNA load was undetectable for 34 % of the DMAS users and 38 % of the control subjects ( P = .49 ) .
	manualset3
256482	4	423972	15	NULL	NULL	NULL	NULL	14 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At week twelve , 38 % of the DMAS users and 14 % of the control subjects had an undetectable plasma HIV RNA load ( P = .014 ) , and at week 24 , the plasma HIV RNA load was undetectable for 34 % of the DMAS users and 38 % of the control subjects ( P = .49 ) .
	manualset3
256483	5	423972	15	NULL	NULL	NULL	NULL	control subjects	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At week twelve , 38 % of the DMAS users and 14 % of the control subjects had an undetectable plasma HIV RNA load ( P = .014 ) , and at week 24 , the plasma HIV RNA load was undetectable for 34 % of the DMAS users and 38 % of the control subjects ( P = .49 ) .
	manualset3
256485	6	423972	15	NULL	NULL	NULL	NULL	plasma HIV RNA load	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At week twelve , 38 % of the DMAS users and 14 % of the control subjects had an undetectable plasma HIV RNA load ( P = .014 ) , and at week 24 , the plasma HIV RNA load was undetectable for 34 % of the DMAS users and 38 % of the control subjects ( P = .49 ) .
	manualset3
256486	7	423972	15	NULL	NULL	NULL	NULL	P = .014	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At week twelve , 38 % of the DMAS users and 14 % of the control subjects had an undetectable plasma HIV RNA load ( P = .014 ) , and at week 24 , the plasma HIV RNA load was undetectable for 34 % of the DMAS users and 38 % of the control subjects ( P = .49 ) .
	manualset3
256487	8	423972	15	NULL	NULL	NULL	NULL	week 24	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At week twelve , 38 % of the DMAS users and 14 % of the control subjects had an undetectable plasma HIV RNA load ( P = .014 ) , and at week 24 , the plasma HIV RNA load was undetectable for 34 % of the DMAS users and 38 % of the control subjects ( P = .49 ) .
	manualset3
256488	9	423972	15	NULL	NULL	NULL	NULL	plasma HIV RNA load	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At week twelve , 38 % of the DMAS users and 14 % of the control subjects had an undetectable plasma HIV RNA load ( P = .014 ) , and at week 24 , the plasma HIV RNA load was undetectable for 34 % of the DMAS users and 38 % of the control subjects ( P = .49 ) .
	manualset3
256489	10	423972	15	NULL	NULL	NULL	NULL	34 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At week twelve , 38 % of the DMAS users and 14 % of the control subjects had an undetectable plasma HIV RNA load ( P = .014 ) , and at week 24 , the plasma HIV RNA load was undetectable for 34 % of the DMAS users and 38 % of the control subjects ( P = .49 ) .
	manualset3
256490	11	423972	15	NULL	NULL	NULL	NULL	DMAS users 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At week twelve , 38 % of the DMAS users and 14 % of the control subjects had an undetectable plasma HIV RNA load ( P = .014 ) , and at week 24 , the plasma HIV RNA load was undetectable for 34 % of the DMAS users and 38 % of the control subjects ( P = .49 ) .
	manualset3
256492	12	423972	15	NULL	NULL	NULL	NULL	38 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At week twelve , 38 % of the DMAS users and 14 % of the control subjects had an undetectable plasma HIV RNA load ( P = .014 ) , and at week 24 , the plasma HIV RNA load was undetectable for 34 % of the DMAS users and 38 % of the control subjects ( P = .49 ) .
	manualset3
256493	13	423972	15	NULL	NULL	NULL	NULL	control subjects 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At week twelve , 38 % of the DMAS users and 14 % of the control subjects had an undetectable plasma HIV RNA load ( P = .014 ) , and at week 24 , the plasma HIV RNA load was undetectable for 34 % of the DMAS users and 38 % of the control subjects ( P = .49 ) .
	manualset3
256495	14	423972	15	NULL	NULL	NULL	NULL	P = .49 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	At week twelve , 38 % of the DMAS users and 14 % of the control subjects had an undetectable plasma HIV RNA load ( P = .014 ) , and at week 24 , the plasma HIV RNA load was undetectable for 34 % of the DMAS users and 38 % of the control subjects ( P = .49 ) .
	manualset3
256500	1	423973	15	NULL	NULL	NULL	NULL	Atenolol treatment 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atenolol treatment reduced REE by 77 + / -14 kcal/day and propranolol by 48 + / -13 kcal/day , respectively ( P & lt ; 0.05 versus pretreatment values ) .
	manualset3
256503	2	423973	15	NULL	NULL	NULL	NULL	REE	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atenolol treatment reduced REE by 77 + / -14 kcal/day and propranolol by 48 + / -13 kcal/day , respectively ( P & lt ; 0.05 versus pretreatment values ) .
	manualset3
256504	3	423973	15	NULL	NULL	NULL	NULL	77 + / -14 kcal/day	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atenolol treatment reduced REE by 77 + / -14 kcal/day and propranolol by 48 + / -13 kcal/day , respectively ( P & lt ; 0.05 versus pretreatment values ) .
	manualset3
256505	4	423973	15	NULL	NULL	NULL	NULL	propranolol	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atenolol treatment reduced REE by 77 + / -14 kcal/day and propranolol by 48 + / -13 kcal/day , respectively ( P & lt ; 0.05 versus pretreatment values ) .
	manualset3
256506	5	423973	15	NULL	NULL	NULL	NULL	48 + / -13 kcal/day	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atenolol treatment reduced REE by 77 + / -14 kcal/day and propranolol by 48 + / -13 kcal/day , respectively ( P & lt ; 0.05 versus pretreatment values ) .
	manualset3
256507	6	423973	15	NULL	NULL	NULL	NULL	P & lt ; 0.05 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atenolol treatment reduced REE by 77 + / -14 kcal/day and propranolol by 48 + / -13 kcal/day , respectively ( P & lt ; 0.05 versus pretreatment values ) .
	manualset3
256508	7	423973	15	NULL	NULL	NULL	NULL	pretreatment values	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atenolol treatment reduced REE by 77 + / -14 kcal/day and propranolol by 48 + / -13 kcal/day , respectively ( P & lt ; 0.05 versus pretreatment values ) .
	manualset3
256509	1	423974	15	NULL	NULL	NULL	NULL	Atherosclerosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atherosclerosis : cell biology and lipoproteins .
	manualset3
256510	2	423974	15	NULL	NULL	NULL	NULL	cell biology	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atherosclerosis : cell biology and lipoproteins .
	manualset3
256511	3	423974	15	NULL	NULL	NULL	NULL	lipoproteins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atherosclerosis : cell biology and lipoproteins .
	manualset3
256512	1	423975	15	NULL	NULL	NULL	NULL	Estrogen	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Estrogen-producing ovarian tumors ) .
	manualset3
256513	2	423975	15	NULL	NULL	NULL	NULL	ovarian tumors	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Estrogen-producing ovarian tumors ) .
	manualset3
256514	1	423976	15	NULL	NULL	NULL	NULL	Atherosclerotic plaques	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atherosclerotic plaques of carotid arteries were detected only in group 2 .
	manualset3
256515	2	423976	15	NULL	NULL	NULL	NULL	carotid arteries	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atherosclerotic plaques of carotid arteries were detected only in group 2 .
	manualset3
256516	3	423976	15	NULL	NULL	NULL	NULL	group 2	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atherosclerotic plaques of carotid arteries were detected only in group 2 .
	manualset3
256517	1	423977	15	NULL	NULL	NULL	NULL	Atomic force microscopy	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atomic force microscopy indicates that the fibrils and their constituent protofilaments have diameters compatible with those of natural amyloid fibrils .
	manualset3
256518	2	423977	15	NULL	NULL	NULL	NULL	fibrils	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atomic force microscopy indicates that the fibrils and their constituent protofilaments have diameters compatible with those of natural amyloid fibrils .
	manualset3
256519	3	423977	15	NULL	NULL	NULL	NULL	constituent protofilaments	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atomic force microscopy indicates that the fibrils and their constituent protofilaments have diameters compatible with those of natural amyloid fibrils .
	manualset3
256520	4	423977	15	NULL	NULL	NULL	NULL	diameters	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atomic force microscopy indicates that the fibrils and their constituent protofilaments have diameters compatible with those of natural amyloid fibrils .
	manualset3
256521	5	423977	15	NULL	NULL	NULL	NULL	natural amyloid fibrils 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atomic force microscopy indicates that the fibrils and their constituent protofilaments have diameters compatible with those of natural amyloid fibrils .
	manualset3
256522	1	423978	15	NULL	NULL	NULL	NULL	Atomic order	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atomic order and magnetization distribution in the half metallic and nearly half metallic C1 ( b ) compounds NiMnSb and PdMnSb .
	manualset3
256523	2	423978	15	NULL	NULL	NULL	NULL	magnetization distribution	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atomic order and magnetization distribution in the half metallic and nearly half metallic C1 ( b ) compounds NiMnSb and PdMnSb .
	manualset3
256524	3	423978	15	NULL	NULL	NULL	NULL	half metallic compounds	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atomic order and magnetization distribution in the half metallic and nearly half metallic C1 ( b ) compounds NiMnSb and PdMnSb .
	manualset3
256525	4	423978	15	NULL	NULL	NULL	NULL	half metallic C1 ( b ) compounds	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atomic order and magnetization distribution in the half metallic and nearly half metallic C1 ( b ) compounds NiMnSb and PdMnSb .
	manualset3
256641	5	423978	15	NULL	NULL	NULL	NULL	NiMnSb	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atomic order and magnetization distribution in the half metallic and nearly half metallic C1 ( b ) compounds NiMnSb and PdMnSb .
	manualset3
256642	6	423978	15	NULL	NULL	NULL	NULL	PdMnSb	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atomic order and magnetization distribution in the half metallic and nearly half metallic C1 ( b ) compounds NiMnSb and PdMnSb .
	manualset3
256536	1	423979	15	NULL	NULL	NULL	NULL	Atomistic MD simulations	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atomistic MD simulations of EHAC , on the other hand , suggest that this membrane is unstable .
	manualset3
256538	2	423979	15	NULL	NULL	NULL	NULL	EHAC	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atomistic MD simulations of EHAC , on the other hand , suggest that this membrane is unstable .
	manualset3
256550	3	423979	15	NULL	NULL	NULL	NULL	membrane	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atomistic MD simulations of EHAC , on the other hand , suggest that this membrane is unstable .
	manualset3
256557	1	423980	15	NULL	NULL	NULL	NULL	Atrial trabeculae	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atrial trabeculae were obtained during coronary bypass surgery .
	manualset3
256560	2	423980	15	NULL	NULL	NULL	NULL	coronary bypass surgery	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atrial trabeculae were obtained during coronary bypass surgery .
	manualset3
256564	1	423981	15	NULL	NULL	NULL	NULL	Atrophy in the thymus 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atrophy in the thymus was significantly increased in all dosed groups of females , except the 0.1 mg/kg group , and in males administered 10 mg/kg or greater .
	manualset3
256566	2	423981	15	NULL	NULL	NULL	NULL	dosed groups of females	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atrophy in the thymus was significantly increased in all dosed groups of females , except the 0.1 mg/kg group , and in males administered 10 mg/kg or greater .
	manualset3
256569	3	423981	15	NULL	NULL	NULL	NULL	0.1 mg/kg group	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atrophy in the thymus was significantly increased in all dosed groups of females , except the 0.1 mg/kg group , and in males administered 10 mg/kg or greater .
	manualset3
256571	4	423981	15	NULL	NULL	NULL	NULL	males	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atrophy in the thymus was significantly increased in all dosed groups of females , except the 0.1 mg/kg group , and in males administered 10 mg/kg or greater .
	manualset3
256573	5	423981	15	NULL	NULL	NULL	NULL	10 mg/kg 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atrophy in the thymus was significantly increased in all dosed groups of females , except the 0.1 mg/kg group , and in males administered 10 mg/kg or greater .
	manualset3
256577	1	423982	15	NULL	NULL	NULL	NULL	Atropine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atropine ( 1 x 10-5 m ) significantly inhibited the effect of BET , whereas pre-incubation with hexamethonium or tetrodotoxin ( TTX ) had no effect , suggesting that the effect was mediated by cholinergic receptors on the smooth muscle .
	manualset3
256578	2	423982	15	NULL	NULL	NULL	NULL	1 x 10-5 m	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atropine ( 1 x 10-5 m ) significantly inhibited the effect of BET , whereas pre-incubation with hexamethonium or tetrodotoxin ( TTX ) had no effect , suggesting that the effect was mediated by cholinergic receptors on the smooth muscle .
	manualset3
256580	3	423982	15	NULL	NULL	NULL	NULL	effect of BET	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atropine ( 1 x 10-5 m ) significantly inhibited the effect of BET , whereas pre-incubation with hexamethonium or tetrodotoxin ( TTX ) had no effect , suggesting that the effect was mediated by cholinergic receptors on the smooth muscle .
	manualset3
256583	4	423982	15	NULL	NULL	NULL	NULL	pre-incubation with hexamethonium	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atropine ( 1 x 10-5 m ) significantly inhibited the effect of BET , whereas pre-incubation with hexamethonium or tetrodotoxin ( TTX ) had no effect , suggesting that the effect was mediated by cholinergic receptors on the smooth muscle .
	manualset3
256587	5	423982	15	NULL	NULL	NULL	NULL	pre-incubation with tetrodotoxin ( TTX ) 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atropine ( 1 x 10-5 m ) significantly inhibited the effect of BET , whereas pre-incubation with hexamethonium or tetrodotoxin ( TTX ) had no effect , suggesting that the effect was mediated by cholinergic receptors on the smooth muscle .
	manualset3
256590	6	423982	15	NULL	NULL	NULL	NULL	effect	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atropine ( 1 x 10-5 m ) significantly inhibited the effect of BET , whereas pre-incubation with hexamethonium or tetrodotoxin ( TTX ) had no effect , suggesting that the effect was mediated by cholinergic receptors on the smooth muscle .
	manualset3
256591	7	423982	15	NULL	NULL	NULL	NULL	effect	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atropine ( 1 x 10-5 m ) significantly inhibited the effect of BET , whereas pre-incubation with hexamethonium or tetrodotoxin ( TTX ) had no effect , suggesting that the effect was mediated by cholinergic receptors on the smooth muscle .
	manualset3
256592	8	423982	15	NULL	NULL	NULL	NULL	cholinergic receptors	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atropine ( 1 x 10-5 m ) significantly inhibited the effect of BET , whereas pre-incubation with hexamethonium or tetrodotoxin ( TTX ) had no effect , suggesting that the effect was mediated by cholinergic receptors on the smooth muscle .
	manualset3
256593	9	423982	15	NULL	NULL	NULL	NULL	smooth muscle	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atropine ( 1 x 10-5 m ) significantly inhibited the effect of BET , whereas pre-incubation with hexamethonium or tetrodotoxin ( TTX ) had no effect , suggesting that the effect was mediated by cholinergic receptors on the smooth muscle .
	manualset3
256600	1	423983	15	NULL	NULL	NULL	NULL	Atropine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atropine , hyoscine butylbromide , or scopolamine are equally effective for the treatment of death rattle in terminal care .
	manualset3
256601	2	423983	15	NULL	NULL	NULL	NULL	hyoscine butylbromide 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atropine , hyoscine butylbromide , or scopolamine are equally effective for the treatment of death rattle in terminal care .
	manualset3
256602	3	423983	15	NULL	NULL	NULL	NULL	scopolamine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atropine , hyoscine butylbromide , or scopolamine are equally effective for the treatment of death rattle in terminal care .
	manualset3
256603	4	423983	15	NULL	NULL	NULL	NULL	treatment of death rattle 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atropine , hyoscine butylbromide , or scopolamine are equally effective for the treatment of death rattle in terminal care .
	manualset3
256604	5	423983	15	NULL	NULL	NULL	NULL	terminal care	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atropine , hyoscine butylbromide , or scopolamine are equally effective for the treatment of death rattle in terminal care .
	manualset3
256605	1	423984	15	NULL	NULL	NULL	NULL	Atropine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atropine increases inspiratory flow during enflurane anaesthesia after pethidine premedication .
	manualset3
256606	2	423984	15	NULL	NULL	NULL	NULL	inspiratory flow	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atropine increases inspiratory flow during enflurane anaesthesia after pethidine premedication .
	manualset3
256607	3	423984	15	NULL	NULL	NULL	NULL	enflurane anaesthesia 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atropine increases inspiratory flow during enflurane anaesthesia after pethidine premedication .
	manualset3
256608	4	423984	15	NULL	NULL	NULL	NULL	pethidine premedication	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atropine increases inspiratory flow during enflurane anaesthesia after pethidine premedication .
	manualset3
256609	1	423985	15	NULL	NULL	NULL	NULL	Atropo-enantioselective total synthesis 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atropo-enantioselective total synthesis of knipholone and related antiplasmodial phenylanthraquinones .
	manualset3
256610	2	423985	15	NULL	NULL	NULL	NULL	 knipholone	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atropo-enantioselective total synthesis of knipholone and related antiplasmodial phenylanthraquinones .
	manualset3
256611	3	423985	15	NULL	NULL	NULL	NULL	antiplasmodial phenylanthraquinones	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atropo-enantioselective total synthesis of knipholone and related antiplasmodial phenylanthraquinones .
	manualset3
256612	1	423986	15	NULL	NULL	NULL	NULL	objectives	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attaining these objectives will be difficult , but less costly than one might suppose , and there is little to be gained by delay .
	manualset3
259731	2	423986	15	NULL	NULL	NULL	NULL	delay	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attaining these objectives will be difficult , but less costly than one might suppose , and there is little to be gained by delay .
	manualset3
256715	1	423987	15	NULL	NULL	NULL	NULL	prophylaxis	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempted passive prophylaxis with a monoclonal anti-Burkholderia pseudomallei exopolysaccharide antibody in a murine model of melioidosis .
	manualset3
256718	2	423987	15	NULL	NULL	NULL	NULL	monoclonal anti-Burkholderia pseudomallei exopolysaccharide antibody	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempted passive prophylaxis with a monoclonal anti-Burkholderia pseudomallei exopolysaccharide antibody in a murine model of melioidosis .
	manualset3
256720	3	423987	15	NULL	NULL	NULL	NULL	murine model	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempted passive prophylaxis with a monoclonal anti-Burkholderia pseudomallei exopolysaccharide antibody in a murine model of melioidosis .
	manualset3
256723	4	423987	15	NULL	NULL	NULL	NULL	melioidosis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempted passive prophylaxis with a monoclonal anti-Burkholderia pseudomallei exopolysaccharide antibody in a murine model of melioidosis .
	manualset3
256729	1	423988	15	NULL	NULL	NULL	NULL	Attempts	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempts at laparoscopic cholecystectomy , however , are more likely to require conversion to an open procedure .
	manualset3
256732	2	423988	15	NULL	NULL	NULL	NULL	laparoscopic cholecystectomy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempts at laparoscopic cholecystectomy , however , are more likely to require conversion to an open procedure .
	manualset3
256735	3	423988	15	NULL	NULL	NULL	NULL	conversion	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempts at laparoscopic cholecystectomy , however , are more likely to require conversion to an open procedure .
	manualset3
256736	4	423988	15	NULL	NULL	NULL	NULL	open procedure	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempts at laparoscopic cholecystectomy , however , are more likely to require conversion to an open procedure .
	manualset3
256738	1	423989	15	NULL	NULL	NULL	NULL	Attempts	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempts have been made to find alpha 1-antagonists that have a selective effect on the prostate ( alfuzosin ) , are long acting ( tamsulosin , terazosin , doxazosin ) or present specificity on the alpha 1A prostatic adrenoceptors ( tamsulosin ) , in order to maintain efficacy without affecting blood pressure .
	manualset3
256740	2	423989	15	NULL	NULL	NULL	NULL	alpha 1-antagonists 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempts have been made to find alpha 1-antagonists that have a selective effect on the prostate ( alfuzosin ) , are long acting ( tamsulosin , terazosin , doxazosin ) or present specificity on the alpha 1A prostatic adrenoceptors ( tamsulosin ) , in order to maintain efficacy without affecting blood pressure .
	manualset3
256743	3	423989	15	NULL	NULL	NULL	NULL	effect	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempts have been made to find alpha 1-antagonists that have a selective effect on the prostate ( alfuzosin ) , are long acting ( tamsulosin , terazosin , doxazosin ) or present specificity on the alpha 1A prostatic adrenoceptors ( tamsulosin ) , in order to maintain efficacy without affecting blood pressure .
	manualset3
256745	4	423989	15	NULL	NULL	NULL	NULL	prostate 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempts have been made to find alpha 1-antagonists that have a selective effect on the prostate ( alfuzosin ) , are long acting ( tamsulosin , terazosin , doxazosin ) or present specificity on the alpha 1A prostatic adrenoceptors ( tamsulosin ) , in order to maintain efficacy without affecting blood pressure .
	manualset3
256747	5	423989	15	NULL	NULL	NULL	NULL	alfuzosin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempts have been made to find alpha 1-antagonists that have a selective effect on the prostate ( alfuzosin ) , are long acting ( tamsulosin , terazosin , doxazosin ) or present specificity on the alpha 1A prostatic adrenoceptors ( tamsulosin ) , in order to maintain efficacy without affecting blood pressure .
	manualset3
256749	6	423989	15	NULL	NULL	NULL	NULL	tamsulosin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempts have been made to find alpha 1-antagonists that have a selective effect on the prostate ( alfuzosin ) , are long acting ( tamsulosin , terazosin , doxazosin ) or present specificity on the alpha 1A prostatic adrenoceptors ( tamsulosin ) , in order to maintain efficacy without affecting blood pressure .
	manualset3
256750	7	423989	15	NULL	NULL	NULL	NULL	terazosin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempts have been made to find alpha 1-antagonists that have a selective effect on the prostate ( alfuzosin ) , are long acting ( tamsulosin , terazosin , doxazosin ) or present specificity on the alpha 1A prostatic adrenoceptors ( tamsulosin ) , in order to maintain efficacy without affecting blood pressure .
	manualset3
256751	8	423989	15	NULL	NULL	NULL	NULL	doxazosin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempts have been made to find alpha 1-antagonists that have a selective effect on the prostate ( alfuzosin ) , are long acting ( tamsulosin , terazosin , doxazosin ) or present specificity on the alpha 1A prostatic adrenoceptors ( tamsulosin ) , in order to maintain efficacy without affecting blood pressure .
	manualset3
256752	9	423989	15	NULL	NULL	NULL	NULL	specificity	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempts have been made to find alpha 1-antagonists that have a selective effect on the prostate ( alfuzosin ) , are long acting ( tamsulosin , terazosin , doxazosin ) or present specificity on the alpha 1A prostatic adrenoceptors ( tamsulosin ) , in order to maintain efficacy without affecting blood pressure .
	manualset3
256754	10	423989	15	NULL	NULL	NULL	NULL	alpha 1A prostatic adrenoceptors	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempts have been made to find alpha 1-antagonists that have a selective effect on the prostate ( alfuzosin ) , are long acting ( tamsulosin , terazosin , doxazosin ) or present specificity on the alpha 1A prostatic adrenoceptors ( tamsulosin ) , in order to maintain efficacy without affecting blood pressure .
	manualset3
256755	11	423989	15	NULL	NULL	NULL	NULL	tamsulosin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempts have been made to find alpha 1-antagonists that have a selective effect on the prostate ( alfuzosin ) , are long acting ( tamsulosin , terazosin , doxazosin ) or present specificity on the alpha 1A prostatic adrenoceptors ( tamsulosin ) , in order to maintain efficacy without affecting blood pressure .
	manualset3
256756	12	423989	15	NULL	NULL	NULL	NULL	efficacy	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempts have been made to find alpha 1-antagonists that have a selective effect on the prostate ( alfuzosin ) , are long acting ( tamsulosin , terazosin , doxazosin ) or present specificity on the alpha 1A prostatic adrenoceptors ( tamsulosin ) , in order to maintain efficacy without affecting blood pressure .
	manualset3
256757	13	423989	15	NULL	NULL	NULL	NULL	blood pressure	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempts have been made to find alpha 1-antagonists that have a selective effect on the prostate ( alfuzosin ) , are long acting ( tamsulosin , terazosin , doxazosin ) or present specificity on the alpha 1A prostatic adrenoceptors ( tamsulosin ) , in order to maintain efficacy without affecting blood pressure .
	manualset3
256770	1	423990	15	NULL	NULL	NULL	NULL	Attempts	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempts to increase the DNA yield from FFPET using WGA were unsuccessful .
	manualset3
256778	2	423990	15	NULL	NULL	NULL	NULL	DNA yield	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempts to increase the DNA yield from FFPET using WGA were unsuccessful .
	manualset3
256780	3	423990	15	NULL	NULL	NULL	NULL	FFPET	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempts to increase the DNA yield from FFPET using WGA were unsuccessful .
	manualset3
256781	4	423990	15	NULL	NULL	NULL	NULL	WGA	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempts to increase the DNA yield from FFPET using WGA were unsuccessful .
	manualset3
256782	1	423991	15	NULL	NULL	NULL	NULL	Attempts	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempts to overcome the dose-limiting toxicity of cisplatin by administering high-dose cisplatin ( 40 mg/m2/d for five days ) in hypertonic saline or with thiosulfate protection are also reviewed .
	manualset3
256783	2	423991	15	NULL	NULL	NULL	NULL	dose-limiting toxicity 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempts to overcome the dose-limiting toxicity of cisplatin by administering high-dose cisplatin ( 40 mg/m2/d for five days ) in hypertonic saline or with thiosulfate protection are also reviewed .
	manualset3
256785	3	423991	15	NULL	NULL	NULL	NULL	cisplatin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempts to overcome the dose-limiting toxicity of cisplatin by administering high-dose cisplatin ( 40 mg/m2/d for five days ) in hypertonic saline or with thiosulfate protection are also reviewed .
	manualset3
256788	4	423991	15	NULL	NULL	NULL	NULL	dose 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempts to overcome the dose-limiting toxicity of cisplatin by administering high-dose cisplatin ( 40 mg/m2/d for five days ) in hypertonic saline or with thiosulfate protection are also reviewed .
	manualset3
256791	5	423991	15	NULL	NULL	NULL	NULL	cisplatin 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempts to overcome the dose-limiting toxicity of cisplatin by administering high-dose cisplatin ( 40 mg/m2/d for five days ) in hypertonic saline or with thiosulfate protection are also reviewed .
	manualset3
256792	6	423991	15	NULL	NULL	NULL	NULL	40 mg/m2/d 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempts to overcome the dose-limiting toxicity of cisplatin by administering high-dose cisplatin ( 40 mg/m2/d for five days ) in hypertonic saline or with thiosulfate protection are also reviewed .
	manualset3
256793	7	423991	15	NULL	NULL	NULL	NULL	five days	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempts to overcome the dose-limiting toxicity of cisplatin by administering high-dose cisplatin ( 40 mg/m2/d for five days ) in hypertonic saline or with thiosulfate protection are also reviewed .
	manualset3
256794	8	423991	15	NULL	NULL	NULL	NULL	hypertonic saline 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempts to overcome the dose-limiting toxicity of cisplatin by administering high-dose cisplatin ( 40 mg/m2/d for five days ) in hypertonic saline or with thiosulfate protection are also reviewed .
	manualset3
256796	9	423991	15	NULL	NULL	NULL	NULL	thiosulfate protection	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attempts to overcome the dose-limiting toxicity of cisplatin by administering high-dose cisplatin ( 40 mg/m2/d for five days ) in hypertonic saline or with thiosulfate protection are also reviewed .
	manualset3
256802	1	423992	15	NULL	NULL	NULL	NULL	Attention-deficit hyperactivity disorder ( ADHD )	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attention-deficit hyperactivity disorder ( ADHD ) is defined as a clinically heterogeneous neurodevelopmental syndrome with the contribution of numerous genetic and environmental risk factors .
	manualset3
256804	2	423992	15	NULL	NULL	NULL	NULL	clinically heterogeneous neurodevelopmental syndrome	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attention-deficit hyperactivity disorder ( ADHD ) is defined as a clinically heterogeneous neurodevelopmental syndrome with the contribution of numerous genetic and environmental risk factors .
	manualset3
256806	3	423992	15	NULL	NULL	NULL	NULL	contribution 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attention-deficit hyperactivity disorder ( ADHD ) is defined as a clinically heterogeneous neurodevelopmental syndrome with the contribution of numerous genetic and environmental risk factors .
	manualset3
256810	4	423992	15	NULL	NULL	NULL	NULL	genetic risk factors 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attention-deficit hyperactivity disorder ( ADHD ) is defined as a clinically heterogeneous neurodevelopmental syndrome with the contribution of numerous genetic and environmental risk factors .
	manualset3
256811	5	423992	15	NULL	NULL	NULL	NULL	environmental risk factors	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attention-deficit hyperactivity disorder ( ADHD ) is defined as a clinically heterogeneous neurodevelopmental syndrome with the contribution of numerous genetic and environmental risk factors .
	manualset3
256815	1	423993	15	NULL	NULL	NULL	NULL	Attention	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attention is also called to disorders in certain neurotransmitting systems ( dopaminergic , acetylcholinergic ) as well as to brain hypometabolism in basal ganglia , thalamus and prefrontal cortex .
	manualset3
256816	2	423993	15	NULL	NULL	NULL	NULL	disorders	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attention is also called to disorders in certain neurotransmitting systems ( dopaminergic , acetylcholinergic ) as well as to brain hypometabolism in basal ganglia , thalamus and prefrontal cortex .
	manualset3
256818	3	423993	15	NULL	NULL	NULL	NULL	neurotransmitting systems	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attention is also called to disorders in certain neurotransmitting systems ( dopaminergic , acetylcholinergic ) as well as to brain hypometabolism in basal ganglia , thalamus and prefrontal cortex .
	manualset3
256821	4	423993	15	NULL	NULL	NULL	NULL	dopaminergic	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attention is also called to disorders in certain neurotransmitting systems ( dopaminergic , acetylcholinergic ) as well as to brain hypometabolism in basal ganglia , thalamus and prefrontal cortex .
	manualset3
256823	5	423993	15	NULL	NULL	NULL	NULL	acetylcholinergic 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attention is also called to disorders in certain neurotransmitting systems ( dopaminergic , acetylcholinergic ) as well as to brain hypometabolism in basal ganglia , thalamus and prefrontal cortex .
	manualset3
256825	6	423993	15	NULL	NULL	NULL	NULL	brain hypometabolism 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attention is also called to disorders in certain neurotransmitting systems ( dopaminergic , acetylcholinergic ) as well as to brain hypometabolism in basal ganglia , thalamus and prefrontal cortex .
	manualset3
256828	7	423993	15	NULL	NULL	NULL	NULL	basal ganglia	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attention is also called to disorders in certain neurotransmitting systems ( dopaminergic , acetylcholinergic ) as well as to brain hypometabolism in basal ganglia , thalamus and prefrontal cortex .
	manualset3
256829	8	423993	15	NULL	NULL	NULL	NULL	thalamus	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attention is also called to disorders in certain neurotransmitting systems ( dopaminergic , acetylcholinergic ) as well as to brain hypometabolism in basal ganglia , thalamus and prefrontal cortex .
	manualset3
256830	9	423993	15	NULL	NULL	NULL	NULL	prefrontal cortex	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attention is also called to disorders in certain neurotransmitting systems ( dopaminergic , acetylcholinergic ) as well as to brain hypometabolism in basal ganglia , thalamus and prefrontal cortex .
	manualset3
256837	1	423994	15	NULL	NULL	NULL	NULL	Attention	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attention is drawn to a mechanism of redox control of gene expression involving Fe-S proteins which depends on the disassembly and reassembly of Fe-S clusters rather than a change in oxidation state .
	manualset3
256840	2	423994	15	NULL	NULL	NULL	NULL	mechanism of redox control 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attention is drawn to a mechanism of redox control of gene expression involving Fe-S proteins which depends on the disassembly and reassembly of Fe-S clusters rather than a change in oxidation state .
	manualset3
256842	3	423994	15	NULL	NULL	NULL	NULL	gene expression 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attention is drawn to a mechanism of redox control of gene expression involving Fe-S proteins which depends on the disassembly and reassembly of Fe-S clusters rather than a change in oxidation state .
	manualset3
256844	4	423994	15	NULL	NULL	NULL	NULL	Fe-S proteins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attention is drawn to a mechanism of redox control of gene expression involving Fe-S proteins which depends on the disassembly and reassembly of Fe-S clusters rather than a change in oxidation state .
	manualset3
256846	5	423994	15	NULL	NULL	NULL	NULL	disassembly of Fe-S clusters	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attention is drawn to a mechanism of redox control of gene expression involving Fe-S proteins which depends on the disassembly and reassembly of Fe-S clusters rather than a change in oxidation state .
	manualset3
256847	6	423994	15	NULL	NULL	NULL	NULL	reassembly of Fe-S clusters	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attention is drawn to a mechanism of redox control of gene expression involving Fe-S proteins which depends on the disassembly and reassembly of Fe-S clusters rather than a change in oxidation state .
	manualset3
256850	7	423994	15	NULL	NULL	NULL	NULL	change in oxidation state	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attention is drawn to a mechanism of redox control of gene expression involving Fe-S proteins which depends on the disassembly and reassembly of Fe-S clusters rather than a change in oxidation state .
	manualset3
256857	1	423995	15	NULL	NULL	NULL	NULL	Attention	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attention must also be paid as to the stage of dissociation at time of surgery .
	manualset3
256866	2	423995	15	NULL	NULL	NULL	NULL	stage of dissociation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attention must also be paid as to the stage of dissociation at time of surgery .
	manualset3
256867	3	423995	15	NULL	NULL	NULL	NULL	time	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attention must also be paid as to the stage of dissociation at time of surgery .
	manualset3
256869	4	423995	15	NULL	NULL	NULL	NULL	surgery	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attention must also be paid as to the stage of dissociation at time of surgery .
	manualset3
256879	1	423996	15	NULL	NULL	NULL	NULL	Attitudes	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attitudes to cancer and cancer prevention : what do people aged 35-54 years think ?
	manualset3
256880	2	423996	15	NULL	NULL	NULL	NULL	cancer	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attitudes to cancer and cancer prevention : what do people aged 35-54 years think ?
	manualset3
256881	3	423996	15	NULL	NULL	NULL	NULL	cancer prevention	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attitudes to cancer and cancer prevention : what do people aged 35-54 years think ?
	manualset3
256882	4	423996	15	NULL	NULL	NULL	NULL	people	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attitudes to cancer and cancer prevention : what do people aged 35-54 years think ?
	manualset3
256884	5	423996	15	NULL	NULL	NULL	NULL	35-54 years 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Attitudes to cancer and cancer prevention : what do people aged 35-54 years think ?
	manualset3
256890	1	423997	15	NULL	NULL	NULL	NULL	Atypical Pott 's disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atypical Pott 's disease : localized infection of the thoracic spine due to Mycobacterium avium-intracellulare in a patient without human immunodeficiency virus infection .
	manualset3
256896	2	423997	15	NULL	NULL	NULL	NULL	localized infection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atypical Pott 's disease : localized infection of the thoracic spine due to Mycobacterium avium-intracellulare in a patient without human immunodeficiency virus infection .
	manualset3
256898	3	423997	15	NULL	NULL	NULL	NULL	thoracic spine	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atypical Pott 's disease : localized infection of the thoracic spine due to Mycobacterium avium-intracellulare in a patient without human immunodeficiency virus infection .
	manualset3
256903	4	423997	15	NULL	NULL	NULL	NULL	Mycobacterium avium-intracellulare	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atypical Pott 's disease : localized infection of the thoracic spine due to Mycobacterium avium-intracellulare in a patient without human immunodeficiency virus infection .
	manualset3
256904	5	423997	15	NULL	NULL	NULL	NULL	patient 	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atypical Pott 's disease : localized infection of the thoracic spine due to Mycobacterium avium-intracellulare in a patient without human immunodeficiency virus infection .
	manualset3
256906	6	423997	15	NULL	NULL	NULL	NULL	human immunodeficiency virus infection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Atypical Pott 's disease : localized infection of the thoracic spine due to Mycobacterium avium-intracellulare in a patient without human immunodeficiency virus infection .
	manualset3
256910	1	423998	15	NULL	NULL	NULL	NULL	Auditory brain-stem responses	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auditory brain-stem responses in blepharospasm .
	manualset3
256912	2	423998	15	NULL	NULL	NULL	NULL	 blepharospasm	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auditory brain-stem responses in blepharospasm .
	manualset3
256916	1	423999	15	NULL	NULL	NULL	NULL	Auditory evoked magnetic fields 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auditory evoked magnetic fields showed prominent bilateral P100m , N250m , P320m and N450m peaks .
	manualset3
256923	2	423999	15	NULL	NULL	NULL	NULL	P100m peaks	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auditory evoked magnetic fields showed prominent bilateral P100m , N250m , P320m and N450m peaks .
	manualset3
256928	3	423999	15	NULL	NULL	NULL	NULL	N250m peaks	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auditory evoked magnetic fields showed prominent bilateral P100m , N250m , P320m and N450m peaks .
	manualset3
256929	4	423999	15	NULL	NULL	NULL	NULL	P320m peaks	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auditory evoked magnetic fields showed prominent bilateral P100m , N250m , P320m and N450m peaks .
	manualset3
256931	5	423999	15	NULL	NULL	NULL	NULL	N450m peaks	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auditory evoked magnetic fields showed prominent bilateral P100m , N250m , P320m and N450m peaks .
	manualset3
256936	1	424000	15	NULL	NULL	NULL	NULL	Etiology	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Etiology , clinical aspects and therapy of allergic rhinitis ) .
	manualset3
256938	2	424000	15	NULL	NULL	NULL	NULL	clinical aspects	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Etiology , clinical aspects and therapy of allergic rhinitis ) .
	manualset3
256939	3	424000	15	NULL	NULL	NULL	NULL	therapy	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Etiology , clinical aspects and therapy of allergic rhinitis ) .
	manualset3
256940	4	424000	15	NULL	NULL	NULL	NULL	allergic rhinitis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Etiology , clinical aspects and therapy of allergic rhinitis ) .
	manualset3
256950	1	424001	15	NULL	NULL	NULL	NULL	Augmentation of gonadotropin-releasing hormone	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Augmentation of gonadotropin-releasing hormone induced follicular growth with exogenous gonadotropins .
	manualset3
256953	2	424001	15	NULL	NULL	NULL	NULL	follicular growth	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Augmentation of gonadotropin-releasing hormone induced follicular growth with exogenous gonadotropins .
	manualset3
256954	3	424001	15	NULL	NULL	NULL	NULL	exogenous gonadotropins 	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Augmentation of gonadotropin-releasing hormone induced follicular growth with exogenous gonadotropins .
	manualset3
256967	1	424002	15	NULL	NULL	NULL	NULL	August 29/October 24 , 1984	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	August 29/October 24 , 1984 An enzymatic assay for the determination of the concentrations of various beta-lactam antibiotics in serum , urine , and cerebrospinal fluid samples is described .
	manualset3
256969	2	424002	15	NULL	NULL	NULL	NULL	enzymatic assay	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	August 29/October 24 , 1984 An enzymatic assay for the determination of the concentrations of various beta-lactam antibiotics in serum , urine , and cerebrospinal fluid samples is described .
	manualset3
256973	3	424002	15	NULL	NULL	NULL	NULL	determination 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	August 29/October 24 , 1984 An enzymatic assay for the determination of the concentrations of various beta-lactam antibiotics in serum , urine , and cerebrospinal fluid samples is described .
	manualset3
256975	4	424002	15	NULL	NULL	NULL	NULL	concentrations	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	August 29/October 24 , 1984 An enzymatic assay for the determination of the concentrations of various beta-lactam antibiotics in serum , urine , and cerebrospinal fluid samples is described .
	manualset3
256979	5	424002	15	NULL	NULL	NULL	NULL	beta-lactam antibiotics	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	August 29/October 24 , 1984 An enzymatic assay for the determination of the concentrations of various beta-lactam antibiotics in serum , urine , and cerebrospinal fluid samples is described .
	manualset3
256986	6	424002	15	NULL	NULL	NULL	NULL	serum samples	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	August 29/October 24 , 1984 An enzymatic assay for the determination of the concentrations of various beta-lactam antibiotics in serum , urine , and cerebrospinal fluid samples is described .
	manualset3
256990	7	424002	15	NULL	NULL	NULL	NULL	urine samples	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	August 29/October 24 , 1984 An enzymatic assay for the determination of the concentrations of various beta-lactam antibiotics in serum , urine , and cerebrospinal fluid samples is described .
	manualset3
256991	8	424002	15	NULL	NULL	NULL	NULL	cerebrospinal fluid samples 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	August 29/October 24 , 1984 An enzymatic assay for the determination of the concentrations of various beta-lactam antibiotics in serum , urine , and cerebrospinal fluid samples is described .
	manualset3
256998	1	424003	15	NULL	NULL	NULL	NULL	Aurora kinase A-specific T-cell receptor gene transfer	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Aurora kinase A-specific T-cell receptor gene transfer redirects T lymphocytes to display effective antileukemia reactivity .
	manualset3
256999	2	424003	15	NULL	NULL	NULL	NULL	T lymphocytes	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Aurora kinase A-specific T-cell receptor gene transfer redirects T lymphocytes to display effective antileukemia reactivity .
	manualset3
257000	3	424003	15	NULL	NULL	NULL	NULL	antileukemia reactivity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Aurora kinase A-specific T-cell receptor gene transfer redirects T lymphocytes to display effective antileukemia reactivity .
	manualset3
257002	1	424004	15	NULL	NULL	NULL	NULL	Austroinulin ( 1 )	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Austroinulin ( 1 ) and most of the flavonoids showed cytotoxicity against HeLa cells , while austroinulin ( 1 ) exhibited a cell cycle inhibition effect at the G1 stage at the concentration of 15.2 microg/mL ( 47.2 microM ) .
	manualset3
257003	2	424004	15	NULL	NULL	NULL	NULL	flavonoids	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Austroinulin ( 1 ) and most of the flavonoids showed cytotoxicity against HeLa cells , while austroinulin ( 1 ) exhibited a cell cycle inhibition effect at the G1 stage at the concentration of 15.2 microg/mL ( 47.2 microM ) .
	manualset3
257004	3	424004	15	NULL	NULL	NULL	NULL	cytotoxicity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Austroinulin ( 1 ) and most of the flavonoids showed cytotoxicity against HeLa cells , while austroinulin ( 1 ) exhibited a cell cycle inhibition effect at the G1 stage at the concentration of 15.2 microg/mL ( 47.2 microM ) .
	manualset3
257005	4	424004	15	NULL	NULL	NULL	NULL	HeLa cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Austroinulin ( 1 ) and most of the flavonoids showed cytotoxicity against HeLa cells , while austroinulin ( 1 ) exhibited a cell cycle inhibition effect at the G1 stage at the concentration of 15.2 microg/mL ( 47.2 microM ) .
	manualset3
257006	5	424004	15	NULL	NULL	NULL	NULL	austroinulin ( 1 ) 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Austroinulin ( 1 ) and most of the flavonoids showed cytotoxicity against HeLa cells , while austroinulin ( 1 ) exhibited a cell cycle inhibition effect at the G1 stage at the concentration of 15.2 microg/mL ( 47.2 microM ) .
	manualset3
257007	6	424004	15	NULL	NULL	NULL	NULL	cell cycle inhibition effect 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Austroinulin ( 1 ) and most of the flavonoids showed cytotoxicity against HeLa cells , while austroinulin ( 1 ) exhibited a cell cycle inhibition effect at the G1 stage at the concentration of 15.2 microg/mL ( 47.2 microM ) .
	manualset3
257008	7	424004	15	NULL	NULL	NULL	NULL	G1 stage 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Austroinulin ( 1 ) and most of the flavonoids showed cytotoxicity against HeLa cells , while austroinulin ( 1 ) exhibited a cell cycle inhibition effect at the G1 stage at the concentration of 15.2 microg/mL ( 47.2 microM ) .
	manualset3
257009	8	424004	15	NULL	NULL	NULL	NULL	concentration	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Austroinulin ( 1 ) and most of the flavonoids showed cytotoxicity against HeLa cells , while austroinulin ( 1 ) exhibited a cell cycle inhibition effect at the G1 stage at the concentration of 15.2 microg/mL ( 47.2 microM ) .
	manualset3
257010	9	424004	15	NULL	NULL	NULL	NULL	15.2 microg/mL	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Austroinulin ( 1 ) and most of the flavonoids showed cytotoxicity against HeLa cells , while austroinulin ( 1 ) exhibited a cell cycle inhibition effect at the G1 stage at the concentration of 15.2 microg/mL ( 47.2 microM ) .
	manualset3
257011	10	424004	15	NULL	NULL	NULL	NULL	47.2 microM	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Austroinulin ( 1 ) and most of the flavonoids showed cytotoxicity against HeLa cells , while austroinulin ( 1 ) exhibited a cell cycle inhibition effect at the G1 stage at the concentration of 15.2 microg/mL ( 47.2 microM ) .
	manualset3
257012	1	424005	15	NULL	NULL	NULL	NULL	living organisms 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Authentic , well preserved living organisms are basic elements for research in the life sciences and biotechnology .
	manualset3
257013	2	424005	15	NULL	NULL	NULL	NULL	elements	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Authentic , well preserved living organisms are basic elements for research in the life sciences and biotechnology .
	manualset3
257014	3	424005	15	NULL	NULL	NULL	NULL	research	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Authentic , well preserved living organisms are basic elements for research in the life sciences and biotechnology .
	manualset3
257015	4	424005	15	NULL	NULL	NULL	NULL	life sciences 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Authentic , well preserved living organisms are basic elements for research in the life sciences and biotechnology .
	manualset3
257016	5	424005	15	NULL	NULL	NULL	NULL	biotechnology 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Authentic , well preserved living organisms are basic elements for research in the life sciences and biotechnology .
	manualset3
257017	1	424006	15	NULL	NULL	NULL	NULL	Authors	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Authors highlight a high incidence of mumps in males ( 68.1 % ) , urban area ( 67.8 % ) , and winter-spring season ( 62 % ) .
	manualset3
257018	2	424006	15	NULL	NULL	NULL	NULL	incidence	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Authors highlight a high incidence of mumps in males ( 68.1 % ) , urban area ( 67.8 % ) , and winter-spring season ( 62 % ) .
	manualset3
257019	3	424006	15	NULL	NULL	NULL	NULL	mumps	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Authors highlight a high incidence of mumps in males ( 68.1 % ) , urban area ( 67.8 % ) , and winter-spring season ( 62 % ) .
	manualset3
257020	4	424006	15	NULL	NULL	NULL	NULL	males 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Authors highlight a high incidence of mumps in males ( 68.1 % ) , urban area ( 67.8 % ) , and winter-spring season ( 62 % ) .
	manualset3
257021	5	424006	15	NULL	NULL	NULL	NULL	68.1 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Authors highlight a high incidence of mumps in males ( 68.1 % ) , urban area ( 67.8 % ) , and winter-spring season ( 62 % ) .
	manualset3
257022	6	424006	15	NULL	NULL	NULL	NULL	urban area 	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Authors highlight a high incidence of mumps in males ( 68.1 % ) , urban area ( 67.8 % ) , and winter-spring season ( 62 % ) .
	manualset3
257023	7	424006	15	NULL	NULL	NULL	NULL	67.8 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Authors highlight a high incidence of mumps in males ( 68.1 % ) , urban area ( 67.8 % ) , and winter-spring season ( 62 % ) .
	manualset3
257024	8	424006	15	NULL	NULL	NULL	NULL	winter-spring season	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Authors highlight a high incidence of mumps in males ( 68.1 % ) , urban area ( 67.8 % ) , and winter-spring season ( 62 % ) .
	manualset3
257025	9	424006	15	NULL	NULL	NULL	NULL	62 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Authors highlight a high incidence of mumps in males ( 68.1 % ) , urban area ( 67.8 % ) , and winter-spring season ( 62 % ) .
	manualset3
257026	1	424007	15	NULL	NULL	NULL	NULL	Authors	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Authors reviewed the articles looking at inclusion criteria , data collection , methodology , assessment methods , and conclusions for validity and relevance to this article .
	manualset3
257027	2	424007	15	NULL	NULL	NULL	NULL	articles 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Authors reviewed the articles looking at inclusion criteria , data collection , methodology , assessment methods , and conclusions for validity and relevance to this article .
	manualset3
257028	3	424007	15	NULL	NULL	NULL	NULL	inclusion criteria	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Authors reviewed the articles looking at inclusion criteria , data collection , methodology , assessment methods , and conclusions for validity and relevance to this article .
	manualset3
257029	4	424007	15	NULL	NULL	NULL	NULL	data collection	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Authors reviewed the articles looking at inclusion criteria , data collection , methodology , assessment methods , and conclusions for validity and relevance to this article .
	manualset3
257030	5	424007	15	NULL	NULL	NULL	NULL	methodology	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Authors reviewed the articles looking at inclusion criteria , data collection , methodology , assessment methods , and conclusions for validity and relevance to this article .
	manualset3
257031	6	424007	15	NULL	NULL	NULL	NULL	assessment methods 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Authors reviewed the articles looking at inclusion criteria , data collection , methodology , assessment methods , and conclusions for validity and relevance to this article .
	manualset3
257032	7	424007	15	NULL	NULL	NULL	NULL	conclusions	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Authors reviewed the articles looking at inclusion criteria , data collection , methodology , assessment methods , and conclusions for validity and relevance to this article .
	manualset3
257033	8	424007	15	NULL	NULL	NULL	NULL	validity	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Authors reviewed the articles looking at inclusion criteria , data collection , methodology , assessment methods , and conclusions for validity and relevance to this article .
	manualset3
257034	9	424007	15	NULL	NULL	NULL	NULL	relevance	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Authors reviewed the articles looking at inclusion criteria , data collection , methodology , assessment methods , and conclusions for validity and relevance to this article .
	manualset3
257035	10	424007	15	NULL	NULL	NULL	NULL	article	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Authors reviewed the articles looking at inclusion criteria , data collection , methodology , assessment methods , and conclusions for validity and relevance to this article .
	manualset3
257036	1	424008	15	NULL	NULL	NULL	NULL	Autistic spectrum disorders	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Autistic spectrum disorders in velo-cardio facial syndrome ( 22q11 .2 deletion ) .
	manualset3
257037	2	424008	15	NULL	NULL	NULL	NULL	velo-cardio facial syndrome	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Autistic spectrum disorders in velo-cardio facial syndrome ( 22q11 .2 deletion ) .
	manualset3
257049	3	424008	15	NULL	NULL	NULL	NULL	22q11 .2 deletion	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Autistic spectrum disorders in velo-cardio facial syndrome ( 22q11 .2 deletion ) .
	manualset3
257050	1	424009	15	NULL	NULL	NULL	NULL	Etiology	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Etiology , clinical features , precipitating factors , type of ventricular dysfunction , length of stay and mortality of 305 patients admitted to hospital because of heart failure ) .
	manualset3
257051	2	424009	15	NULL	NULL	NULL	NULL	clinical features 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Etiology , clinical features , precipitating factors , type of ventricular dysfunction , length of stay and mortality of 305 patients admitted to hospital because of heart failure ) .
	manualset3
257052	3	424009	15	NULL	NULL	NULL	NULL	precipitating factors	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Etiology , clinical features , precipitating factors , type of ventricular dysfunction , length of stay and mortality of 305 patients admitted to hospital because of heart failure ) .
	manualset3
257053	4	424009	15	NULL	NULL	NULL	NULL	type of ventricular dysfunction	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Etiology , clinical features , precipitating factors , type of ventricular dysfunction , length of stay and mortality of 305 patients admitted to hospital because of heart failure ) .
	manualset3
257054	5	424009	15	NULL	NULL	NULL	NULL	length of stay	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Etiology , clinical features , precipitating factors , type of ventricular dysfunction , length of stay and mortality of 305 patients admitted to hospital because of heart failure ) .
	manualset3
257055	6	424009	15	NULL	NULL	NULL	NULL	mortality	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Etiology , clinical features , precipitating factors , type of ventricular dysfunction , length of stay and mortality of 305 patients admitted to hospital because of heart failure ) .
	manualset3
257056	7	424009	15	NULL	NULL	NULL	NULL	305 patients 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Etiology , clinical features , precipitating factors , type of ventricular dysfunction , length of stay and mortality of 305 patients admitted to hospital because of heart failure ) .
	manualset3
257057	8	424009	15	NULL	NULL	NULL	NULL	hospital	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Etiology , clinical features , precipitating factors , type of ventricular dysfunction , length of stay and mortality of 305 patients admitted to hospital because of heart failure ) .
	manualset3
257058	9	424009	15	NULL	NULL	NULL	NULL	heart failure	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Etiology , clinical features , precipitating factors , type of ventricular dysfunction , length of stay and mortality of 305 patients admitted to hospital because of heart failure ) .
	manualset3
257059	1	424010	15	NULL	NULL	NULL	NULL	Autoimmunity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Autoimmunity may result from an intrinsically abnormal immune system , primary alterations of the target beta cell or both .
	manualset3
257060	2	424010	15	NULL	NULL	NULL	NULL	abnormal immune system	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Autoimmunity may result from an intrinsically abnormal immune system , primary alterations of the target beta cell or both .
	manualset3
257061	3	424010	15	NULL	NULL	NULL	NULL	primary alterations of the target beta cell	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Autoimmunity may result from an intrinsically abnormal immune system , primary alterations of the target beta cell or both .
	manualset3
257062	1	424011	15	NULL	NULL	NULL	NULL	Automated striatal uptake analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Automated striatal uptake analysis of F-FDOPA PET images applied to Parkinson 's disease patients .
	manualset3
257063	2	424011	15	NULL	NULL	NULL	NULL	F-FDOPA PET images	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Automated striatal uptake analysis of F-FDOPA PET images applied to Parkinson 's disease patients .
	manualset3
257064	3	424011	15	NULL	NULL	NULL	NULL	Parkinson 's disease patients 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Automated striatal uptake analysis of F-FDOPA PET images applied to Parkinson 's disease patients .
	manualset3
257065	1	424012	15	NULL	NULL	NULL	NULL	Automated synthesis	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Automated synthesis of the generic peptide labeling agent N-succinimidyl 4 - ( ( 18 ) F ) fluorobenzoate and application to ( 18 ) F-label the vasoactive transmitter urotensin-II as a ligand for positron emission tomography .
	manualset3
257067	2	424012	15	NULL	NULL	NULL	NULL	generic peptide labeling agent N-succinimidyl 4 - ( ( 18 ) F ) fluorobenzoate 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Automated synthesis of the generic peptide labeling agent N-succinimidyl 4 - ( ( 18 ) F ) fluorobenzoate and application to ( 18 ) F-label the vasoactive transmitter urotensin-II as a ligand for positron emission tomography .
	manualset3
257068	3	424012	15	NULL	NULL	NULL	NULL	application to ( 18 ) F-label	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Automated synthesis of the generic peptide labeling agent N-succinimidyl 4 - ( ( 18 ) F ) fluorobenzoate and application to ( 18 ) F-label the vasoactive transmitter urotensin-II as a ligand for positron emission tomography .
	manualset3
257069	4	424012	15	NULL	NULL	NULL	NULL	vasoactive transmitter urotensin-II 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Automated synthesis of the generic peptide labeling agent N-succinimidyl 4 - ( ( 18 ) F ) fluorobenzoate and application to ( 18 ) F-label the vasoactive transmitter urotensin-II as a ligand for positron emission tomography .
	manualset3
257071	5	424012	15	NULL	NULL	NULL	NULL	ligand 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Automated synthesis of the generic peptide labeling agent N-succinimidyl 4 - ( ( 18 ) F ) fluorobenzoate and application to ( 18 ) F-label the vasoactive transmitter urotensin-II as a ligand for positron emission tomography .
	manualset3
257072	6	424012	15	NULL	NULL	NULL	NULL	positron emission tomography	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Automated synthesis of the generic peptide labeling agent N-succinimidyl 4 - ( ( 18 ) F ) fluorobenzoate and application to ( 18 ) F-label the vasoactive transmitter urotensin-II as a ligand for positron emission tomography .
	manualset3
257073	1	424013	15	NULL	NULL	NULL	NULL	Automatic toxic granulation detection	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Automatic toxic granulation detection and grading based on speeded up robust features .
	manualset3
257074	2	424013	15	NULL	NULL	NULL	NULL	grading	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Automatic toxic granulation detection and grading based on speeded up robust features .
	manualset3
257075	3	424013	15	NULL	NULL	NULL	NULL	speeded up robust features	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Automatic toxic granulation detection and grading based on speeded up robust features .
	manualset3
257076	1	424014	15	NULL	NULL	NULL	NULL	Autonomic pain	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Autonomic pain : features and methods of assessment .
	manualset3
257077	2	424014	15	NULL	NULL	NULL	NULL	features of assessment 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Autonomic pain : features and methods of assessment .
	manualset3
257078	3	424014	15	NULL	NULL	NULL	NULL	methods of assessment	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Autonomic pain : features and methods of assessment .
	manualset3
257079	1	424015	15	NULL	NULL	NULL	NULL	contribution	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( A contribution to the immunity of man in ornithosis transmitted by ducks ) .
	manualset3
257080	2	424015	15	NULL	NULL	NULL	NULL	immunity of man	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( A contribution to the immunity of man in ornithosis transmitted by ducks ) .
	manualset3
257081	3	424015	15	NULL	NULL	NULL	NULL	ornithosis 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( A contribution to the immunity of man in ornithosis transmitted by ducks ) .
	manualset3
257082	4	424015	15	NULL	NULL	NULL	NULL	ducks 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( A contribution to the immunity of man in ornithosis transmitted by ducks ) .
	manualset3
257083	1	424016	15	NULL	NULL	NULL	NULL	Autophagy	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Autophagy is an elementary process participating in several cellular events such as cellular clearance and nonapoptotic programmed cell death .
	manualset3
257084	2	424016	15	NULL	NULL	NULL	NULL	elementary process 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Autophagy is an elementary process participating in several cellular events such as cellular clearance and nonapoptotic programmed cell death .
	manualset3
257085	3	424016	15	NULL	NULL	NULL	NULL	cellular events	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Autophagy is an elementary process participating in several cellular events such as cellular clearance and nonapoptotic programmed cell death .
	manualset3
257086	4	424016	15	NULL	NULL	NULL	NULL	cellular clearance 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Autophagy is an elementary process participating in several cellular events such as cellular clearance and nonapoptotic programmed cell death .
	manualset3
257087	5	424016	15	NULL	NULL	NULL	NULL	nonapoptotic programmed cell death	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Autophagy is an elementary process participating in several cellular events such as cellular clearance and nonapoptotic programmed cell death .
	manualset3
257351	1	424017	15	NULL	NULL	NULL	NULL	Autoradiographic bands 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Autoradiographic bands were displaced with IGF-I but not with equimolar levels of IGF-II or insulin .
	manualset3
257353	2	424017	15	NULL	NULL	NULL	NULL	IGF-I	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Autoradiographic bands were displaced with IGF-I but not with equimolar levels of IGF-II or insulin .
	manualset3
257355	3	424017	15	NULL	NULL	NULL	NULL	equimolar levels 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Autoradiographic bands were displaced with IGF-I but not with equimolar levels of IGF-II or insulin .
	manualset3
257357	4	424017	15	NULL	NULL	NULL	NULL	IGF-II 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Autoradiographic bands were displaced with IGF-I but not with equimolar levels of IGF-II or insulin .
	manualset3
257359	5	424017	15	NULL	NULL	NULL	NULL	insulin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Autoradiographic bands were displaced with IGF-I but not with equimolar levels of IGF-II or insulin .
	manualset3
257366	1	424018	15	NULL	NULL	NULL	NULL	Autosomal dominant tauopathy	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Autosomal dominant tauopathy with parkinsonism and central hypoventilation .
	manualset3
257367	2	424018	15	NULL	NULL	NULL	NULL	parkinsonism	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Autosomal dominant tauopathy with parkinsonism and central hypoventilation .
	manualset3
257368	3	424018	15	NULL	NULL	NULL	NULL	central hypoventilation 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Autosomal dominant tauopathy with parkinsonism and central hypoventilation .
	manualset3
257374	1	424019	15	NULL	NULL	NULL	NULL	Autotransfusion 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Autotransfusion : the use of washed red cells as an adjunct to component therapy .
	manualset3
257375	2	424019	15	NULL	NULL	NULL	NULL	red cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Autotransfusion : the use of washed red cells as an adjunct to component therapy .
	manualset3
257393	3	424019	15	NULL	NULL	NULL	NULL	adjunct	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Autotransfusion : the use of washed red cells as an adjunct to component therapy .
	manualset3
257394	4	424019	15	NULL	NULL	NULL	NULL	component therapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Autotransfusion : the use of washed red cells as an adjunct to component therapy .
	manualset3
257395	1	424020	15	NULL	NULL	NULL	NULL	Auxin-induced growth	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auxin-induced growth can be inhibited by scavengers of ROS or inhibitors interfering with the formation of these molecules in the cell wall .
	manualset3
257396	2	424020	15	NULL	NULL	NULL	NULL	scavengers of ROS	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auxin-induced growth can be inhibited by scavengers of ROS or inhibitors interfering with the formation of these molecules in the cell wall .
	manualset3
257397	3	424020	15	NULL	NULL	NULL	NULL	inhibitors	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auxin-induced growth can be inhibited by scavengers of ROS or inhibitors interfering with the formation of these molecules in the cell wall .
	manualset3
257398	4	424020	15	NULL	NULL	NULL	NULL	formation of these molecules	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auxin-induced growth can be inhibited by scavengers of ROS or inhibitors interfering with the formation of these molecules in the cell wall .
	manualset3
257399	5	424020	15	NULL	NULL	NULL	NULL	cell wall	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auxin-induced growth can be inhibited by scavengers of ROS or inhibitors interfering with the formation of these molecules in the cell wall .
	manualset3
257400	1	424021	15	NULL	NULL	NULL	NULL	Auxin signaling	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auxin signaling for differentiation of distal stem cells requires the transcriptional repressor IAA17/AXR3 as well as the ARF10 and ARF16 auxin response factors .
	manualset3
257401	2	424021	15	NULL	NULL	NULL	NULL	differentiation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auxin signaling for differentiation of distal stem cells requires the transcriptional repressor IAA17/AXR3 as well as the ARF10 and ARF16 auxin response factors .
	manualset3
257402	3	424021	15	NULL	NULL	NULL	NULL	distal stem cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auxin signaling for differentiation of distal stem cells requires the transcriptional repressor IAA17/AXR3 as well as the ARF10 and ARF16 auxin response factors .
	manualset3
257403	4	424021	15	NULL	NULL	NULL	NULL	transcriptional repressor IAA17/AXR3 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auxin signaling for differentiation of distal stem cells requires the transcriptional repressor IAA17/AXR3 as well as the ARF10 and ARF16 auxin response factors .
	manualset3
257404	5	424021	15	NULL	NULL	NULL	NULL	ARF10 auxin response factors	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auxin signaling for differentiation of distal stem cells requires the transcriptional repressor IAA17/AXR3 as well as the ARF10 and ARF16 auxin response factors .
	manualset3
257405	6	424021	15	NULL	NULL	NULL	NULL	ARF16 auxin response factors	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auxin signaling for differentiation of distal stem cells requires the transcriptional repressor IAA17/AXR3 as well as the ARF10 and ARF16 auxin response factors .
	manualset3
257406	1	424022	15	NULL	NULL	NULL	NULL	Evaluation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Evaluation of biomaterial surfaces by detection of mechanical and electrical inhomogeneities using scanning probe microscopy ) .
	manualset3
257407	2	424022	15	NULL	NULL	NULL	NULL	biomaterial surfaces 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Evaluation of biomaterial surfaces by detection of mechanical and electrical inhomogeneities using scanning probe microscopy ) .
	manualset3
257408	3	424022	15	NULL	NULL	NULL	NULL	detection of mechanical inhomogeneities 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Evaluation of biomaterial surfaces by detection of mechanical and electrical inhomogeneities using scanning probe microscopy ) .
	manualset3
257409	4	424022	15	NULL	NULL	NULL	NULL	detection of electrical inhomogeneities	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Evaluation of biomaterial surfaces by detection of mechanical and electrical inhomogeneities using scanning probe microscopy ) .
	manualset3
257410	5	424022	15	NULL	NULL	NULL	NULL	scanning probe microscopy	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Evaluation of biomaterial surfaces by detection of mechanical and electrical inhomogeneities using scanning probe microscopy ) .
	manualset3
257415	1	424023	15	NULL	NULL	NULL	NULL	Auxotonic responses	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auxotonic responses were measured in longitudinal muscle strips from the gastric fundus of reserpinized rats ( 5 mg/kg i.p. , 24 hr before sacrifice ) , suspended between parallel platinum electrodes in Krebs solution containing atropine ( 1 microM ) and 5-hydroxytryptamine ( 3 microM ) .
	manualset3
257416	2	424023	15	NULL	NULL	NULL	NULL	longitudinal muscle strips 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auxotonic responses were measured in longitudinal muscle strips from the gastric fundus of reserpinized rats ( 5 mg/kg i.p. , 24 hr before sacrifice ) , suspended between parallel platinum electrodes in Krebs solution containing atropine ( 1 microM ) and 5-hydroxytryptamine ( 3 microM ) .
	manualset3
257417	3	424023	15	NULL	NULL	NULL	NULL	gastric fundus	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auxotonic responses were measured in longitudinal muscle strips from the gastric fundus of reserpinized rats ( 5 mg/kg i.p. , 24 hr before sacrifice ) , suspended between parallel platinum electrodes in Krebs solution containing atropine ( 1 microM ) and 5-hydroxytryptamine ( 3 microM ) .
	manualset3
257418	4	424023	15	NULL	NULL	NULL	NULL	rats 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auxotonic responses were measured in longitudinal muscle strips from the gastric fundus of reserpinized rats ( 5 mg/kg i.p. , 24 hr before sacrifice ) , suspended between parallel platinum electrodes in Krebs solution containing atropine ( 1 microM ) and 5-hydroxytryptamine ( 3 microM ) .
	manualset3
257419	5	424023	15	NULL	NULL	NULL	NULL	5 mg/kg	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auxotonic responses were measured in longitudinal muscle strips from the gastric fundus of reserpinized rats ( 5 mg/kg i.p. , 24 hr before sacrifice ) , suspended between parallel platinum electrodes in Krebs solution containing atropine ( 1 microM ) and 5-hydroxytryptamine ( 3 microM ) .
	manualset3
257420	6	424023	15	NULL	NULL	NULL	NULL	 24 hr before sacrifice	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auxotonic responses were measured in longitudinal muscle strips from the gastric fundus of reserpinized rats ( 5 mg/kg i.p. , 24 hr before sacrifice ) , suspended between parallel platinum electrodes in Krebs solution containing atropine ( 1 microM ) and 5-hydroxytryptamine ( 3 microM ) .
	manualset3
257421	7	424023	15	NULL	NULL	NULL	NULL	parallel platinum electrodes	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auxotonic responses were measured in longitudinal muscle strips from the gastric fundus of reserpinized rats ( 5 mg/kg i.p. , 24 hr before sacrifice ) , suspended between parallel platinum electrodes in Krebs solution containing atropine ( 1 microM ) and 5-hydroxytryptamine ( 3 microM ) .
	manualset3
257422	8	424023	15	NULL	NULL	NULL	NULL	Krebs solution	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auxotonic responses were measured in longitudinal muscle strips from the gastric fundus of reserpinized rats ( 5 mg/kg i.p. , 24 hr before sacrifice ) , suspended between parallel platinum electrodes in Krebs solution containing atropine ( 1 microM ) and 5-hydroxytryptamine ( 3 microM ) .
	manualset3
257423	9	424023	15	NULL	NULL	NULL	NULL	atropine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auxotonic responses were measured in longitudinal muscle strips from the gastric fundus of reserpinized rats ( 5 mg/kg i.p. , 24 hr before sacrifice ) , suspended between parallel platinum electrodes in Krebs solution containing atropine ( 1 microM ) and 5-hydroxytryptamine ( 3 microM ) .
	manualset3
257424	10	424023	15	NULL	NULL	NULL	NULL	1 microM	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auxotonic responses were measured in longitudinal muscle strips from the gastric fundus of reserpinized rats ( 5 mg/kg i.p. , 24 hr before sacrifice ) , suspended between parallel platinum electrodes in Krebs solution containing atropine ( 1 microM ) and 5-hydroxytryptamine ( 3 microM ) .
	manualset3
257425	11	424023	15	NULL	NULL	NULL	NULL	5-hydroxytryptamine	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auxotonic responses were measured in longitudinal muscle strips from the gastric fundus of reserpinized rats ( 5 mg/kg i.p. , 24 hr before sacrifice ) , suspended between parallel platinum electrodes in Krebs solution containing atropine ( 1 microM ) and 5-hydroxytryptamine ( 3 microM ) .
	manualset3
257426	12	424023	15	NULL	NULL	NULL	NULL	3 microM	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Auxotonic responses were measured in longitudinal muscle strips from the gastric fundus of reserpinized rats ( 5 mg/kg i.p. , 24 hr before sacrifice ) , suspended between parallel platinum electrodes in Krebs solution containing atropine ( 1 microM ) and 5-hydroxytryptamine ( 3 microM ) .
	manualset3
257427	1	424024	15	NULL	NULL	NULL	NULL	Availability	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Availability of home sleep diagnostic systems .
	manualset3
257428	2	424024	15	NULL	NULL	NULL	NULL	home sleep diagnostic systems	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Availability of home sleep diagnostic systems .
	manualset3
257461	1	424025	15	NULL	NULL	NULL	NULL	alpha-amino groups	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Available alpha-amino groups decreased with proteinase-negative variants .
	manualset3
257462	2	424025	15	NULL	NULL	NULL	NULL	proteinase-negative variants	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Available alpha-amino groups decreased with proteinase-negative variants .
	manualset3
257463	1	424026	15	NULL	NULL	NULL	NULL	data	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Available are original data on rhinomanometry in children with nasal septum distortion in the anterior part .
	manualset3
257464	2	424026	15	NULL	NULL	NULL	NULL	rhinomanometry	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Available are original data on rhinomanometry in children with nasal septum distortion in the anterior part .
	manualset3
257465	3	424026	15	NULL	NULL	NULL	NULL	children	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Available are original data on rhinomanometry in children with nasal septum distortion in the anterior part .
	manualset3
257466	4	424026	15	NULL	NULL	NULL	NULL	nasal septum distortion	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Available are original data on rhinomanometry in children with nasal septum distortion in the anterior part .
	manualset3
257467	5	424026	15	NULL	NULL	NULL	NULL	anterior part	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Available are original data on rhinomanometry in children with nasal septum distortion in the anterior part .
	manualset3
257468	1	424027	15	NULL	NULL	NULL	NULL	Average MLC reactions 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Average MLC reactions of maternal cells with paternal and control cells were not significantly different , nor did the MLC responses of maternal cells clearly differ from those of other cells in their time-course kinetics .
	manualset3
257469	2	424027	15	NULL	NULL	NULL	NULL	maternal cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Average MLC reactions of maternal cells with paternal and control cells were not significantly different , nor did the MLC responses of maternal cells clearly differ from those of other cells in their time-course kinetics .
	manualset3
257470	3	424027	15	NULL	NULL	NULL	NULL	paternal cells 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Average MLC reactions of maternal cells with paternal and control cells were not significantly different , nor did the MLC responses of maternal cells clearly differ from those of other cells in their time-course kinetics .
	manualset3
257471	4	424027	15	NULL	NULL	NULL	NULL	control cells 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Average MLC reactions of maternal cells with paternal and control cells were not significantly different , nor did the MLC responses of maternal cells clearly differ from those of other cells in their time-course kinetics .
	manualset3
257472	5	424027	15	NULL	NULL	NULL	NULL	MLC responses	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Average MLC reactions of maternal cells with paternal and control cells were not significantly different , nor did the MLC responses of maternal cells clearly differ from those of other cells in their time-course kinetics .
	manualset3
257473	6	424027	15	NULL	NULL	NULL	NULL	maternal cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Average MLC reactions of maternal cells with paternal and control cells were not significantly different , nor did the MLC responses of maternal cells clearly differ from those of other cells in their time-course kinetics .
	manualset3
257474	7	424027	15	NULL	NULL	NULL	NULL	cells 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Average MLC reactions of maternal cells with paternal and control cells were not significantly different , nor did the MLC responses of maternal cells clearly differ from those of other cells in their time-course kinetics .
	manualset3
257475	8	424027	15	NULL	NULL	NULL	NULL	time-course kinetics	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Average MLC reactions of maternal cells with paternal and control cells were not significantly different , nor did the MLC responses of maternal cells clearly differ from those of other cells in their time-course kinetics .
	manualset3
257476	1	424028	15	NULL	NULL	NULL	NULL	Average mf prevalence 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Average mf prevalence in warmer , relatively drier areas receiving 25 mm of rain was significantly higher ( 3.9 % ) than that in less warmer but more humid areas receiving 50 mm of rain ( 1.6 % ) ( P & lt ; 0.0001 ) .
	manualset3
257477	2	424028	15	NULL	NULL	NULL	NULL	areas 	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Average mf prevalence in warmer , relatively drier areas receiving 25 mm of rain was significantly higher ( 3.9 % ) than that in less warmer but more humid areas receiving 50 mm of rain ( 1.6 % ) ( P & lt ; 0.0001 ) .
	manualset3
257478	3	424028	15	NULL	NULL	NULL	NULL	25 mm 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Average mf prevalence in warmer , relatively drier areas receiving 25 mm of rain was significantly higher ( 3.9 % ) than that in less warmer but more humid areas receiving 50 mm of rain ( 1.6 % ) ( P & lt ; 0.0001 ) .
	manualset3
257479	4	424028	15	NULL	NULL	NULL	NULL	rain	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Average mf prevalence in warmer , relatively drier areas receiving 25 mm of rain was significantly higher ( 3.9 % ) than that in less warmer but more humid areas receiving 50 mm of rain ( 1.6 % ) ( P & lt ; 0.0001 ) .
	manualset3
257480	5	424028	15	NULL	NULL	NULL	NULL	3.9 % 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Average mf prevalence in warmer , relatively drier areas receiving 25 mm of rain was significantly higher ( 3.9 % ) than that in less warmer but more humid areas receiving 50 mm of rain ( 1.6 % ) ( P & lt ; 0.0001 ) .
	manualset3
257481	6	424028	15	NULL	NULL	NULL	NULL	humid areas	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Average mf prevalence in warmer , relatively drier areas receiving 25 mm of rain was significantly higher ( 3.9 % ) than that in less warmer but more humid areas receiving 50 mm of rain ( 1.6 % ) ( P & lt ; 0.0001 ) .
	manualset3
257482	7	424028	15	NULL	NULL	NULL	NULL	50 mm	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Average mf prevalence in warmer , relatively drier areas receiving 25 mm of rain was significantly higher ( 3.9 % ) than that in less warmer but more humid areas receiving 50 mm of rain ( 1.6 % ) ( P & lt ; 0.0001 ) .
	manualset3
257483	8	424028	15	NULL	NULL	NULL	NULL	rain 	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Average mf prevalence in warmer , relatively drier areas receiving 25 mm of rain was significantly higher ( 3.9 % ) than that in less warmer but more humid areas receiving 50 mm of rain ( 1.6 % ) ( P & lt ; 0.0001 ) .
	manualset3
257484	9	424028	15	NULL	NULL	NULL	NULL	1.6 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Average mf prevalence in warmer , relatively drier areas receiving 25 mm of rain was significantly higher ( 3.9 % ) than that in less warmer but more humid areas receiving 50 mm of rain ( 1.6 % ) ( P & lt ; 0.0001 ) .
	manualset3
257485	10	424028	15	NULL	NULL	NULL	NULL	P & lt ; 0.0001	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Average mf prevalence in warmer , relatively drier areas receiving 25 mm of rain was significantly higher ( 3.9 % ) than that in less warmer but more humid areas receiving 50 mm of rain ( 1.6 % ) ( P & lt ; 0.0001 ) .
	manualset3
257486	1	424029	15	NULL	NULL	NULL	NULL	Average number 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Average number of rituximab infusions administered to patients was 3.4 cycles .
	manualset3
257487	2	424029	15	NULL	NULL	NULL	NULL	rituximab infusions	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Average number of rituximab infusions administered to patients was 3.4 cycles .
	manualset3
257488	3	424029	15	NULL	NULL	NULL	NULL	patients 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Average number of rituximab infusions administered to patients was 3.4 cycles .
	manualset3
257490	4	424029	15	NULL	NULL	NULL	NULL	3.4 cycles	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Average number of rituximab infusions administered to patients was 3.4 cycles .
	manualset3
257493	1	424030	15	NULL	NULL	NULL	NULL	Average pellet size	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Average pellet size varied between 2.82 x10 ( 5 ) microm ( 3 ) for Paracalanus sp .
	manualset3
257494	2	424030	15	NULL	NULL	NULL	NULL	2.82 x10 ( 5 ) microm ( 3 ) 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Average pellet size varied between 2.82 x10 ( 5 ) microm ( 3 ) for Paracalanus sp .
	manualset3
257496	3	424030	15	NULL	NULL	NULL	NULL	Paracalanus sp	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Average pellet size varied between 2.82 x10 ( 5 ) microm ( 3 ) for Paracalanus sp .
	manualset3
257498	1	424031	15	NULL	NULL	NULL	NULL	changes	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Averaging and Wiener filtering were used to detect changes in tonic EMG activity evoked by dorsiflexing or plantarflexing displacements of the ankle .
	manualset3
257503	2	424031	15	NULL	NULL	NULL	NULL	tonic EMG activity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Averaging and Wiener filtering were used to detect changes in tonic EMG activity evoked by dorsiflexing or plantarflexing displacements of the ankle .
	manualset3
257506	3	424031	15	NULL	NULL	NULL	NULL	dorsiflexing displacements	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Averaging and Wiener filtering were used to detect changes in tonic EMG activity evoked by dorsiflexing or plantarflexing displacements of the ankle .
	manualset3
257507	4	424031	15	NULL	NULL	NULL	NULL	plantarflexing displacements 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Averaging and Wiener filtering were used to detect changes in tonic EMG activity evoked by dorsiflexing or plantarflexing displacements of the ankle .
	manualset3
257509	5	424031	15	NULL	NULL	NULL	NULL	ankle	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Averaging and Wiener filtering were used to detect changes in tonic EMG activity evoked by dorsiflexing or plantarflexing displacements of the ankle .
	manualset3
257512	1	424032	15	NULL	NULL	NULL	NULL	n = 256 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Averaging ( n = 256 , 1024 ms ) centered around the onset of the first lick at the newly contacted spout showed 2-3 lick related potentials in the post-transitional interval whereas only one such wave occasionally appeared at the end of the pre-transition period .
	manualset3
257513	2	424032	15	NULL	NULL	NULL	NULL	1024 ms	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Averaging ( n = 256 , 1024 ms ) centered around the onset of the first lick at the newly contacted spout showed 2-3 lick related potentials in the post-transitional interval whereas only one such wave occasionally appeared at the end of the pre-transition period .
	manualset3
257514	3	424032	15	NULL	NULL	NULL	NULL	onset of the first lick	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Averaging ( n = 256 , 1024 ms ) centered around the onset of the first lick at the newly contacted spout showed 2-3 lick related potentials in the post-transitional interval whereas only one such wave occasionally appeared at the end of the pre-transition period .
	manualset3
257518	4	424032	15	NULL	NULL	NULL	NULL	newly contacted spout	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Averaging ( n = 256 , 1024 ms ) centered around the onset of the first lick at the newly contacted spout showed 2-3 lick related potentials in the post-transitional interval whereas only one such wave occasionally appeared at the end of the pre-transition period .
	manualset3
257519	5	424032	15	NULL	NULL	NULL	NULL	2-3 lick related potentials	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Averaging ( n = 256 , 1024 ms ) centered around the onset of the first lick at the newly contacted spout showed 2-3 lick related potentials in the post-transitional interval whereas only one such wave occasionally appeared at the end of the pre-transition period .
	manualset3
257520	6	424032	15	NULL	NULL	NULL	NULL	post-transitional interval 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Averaging ( n = 256 , 1024 ms ) centered around the onset of the first lick at the newly contacted spout showed 2-3 lick related potentials in the post-transitional interval whereas only one such wave occasionally appeared at the end of the pre-transition period .
	manualset3
257521	7	424032	15	NULL	NULL	NULL	NULL	one 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Averaging ( n = 256 , 1024 ms ) centered around the onset of the first lick at the newly contacted spout showed 2-3 lick related potentials in the post-transitional interval whereas only one such wave occasionally appeared at the end of the pre-transition period .
	manualset3
257522	8	424032	15	NULL	NULL	NULL	NULL	wave	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Averaging ( n = 256 , 1024 ms ) centered around the onset of the first lick at the newly contacted spout showed 2-3 lick related potentials in the post-transitional interval whereas only one such wave occasionally appeared at the end of the pre-transition period .
	manualset3
257524	9	424032	15	NULL	NULL	NULL	NULL	end 	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Averaging ( n = 256 , 1024 ms ) centered around the onset of the first lick at the newly contacted spout showed 2-3 lick related potentials in the post-transitional interval whereas only one such wave occasionally appeared at the end of the pre-transition period .
	manualset3
257525	10	424032	15	NULL	NULL	NULL	NULL	pre-transition period	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Averaging ( n = 256 , 1024 ms ) centered around the onset of the first lick at the newly contacted spout showed 2-3 lick related potentials in the post-transitional interval whereas only one such wave occasionally appeared at the end of the pre-transition period .
	manualset3
257559	1	424033	15	NULL	NULL	NULL	NULL	Avian Influenza A virus polymerase	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Avian Influenza A virus polymerase association with nucleoprotein , but not polymerase assembly , is impaired in human cells during the course of infection .
	manualset3
257561	2	424033	15	NULL	NULL	NULL	NULL	association 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Avian Influenza A virus polymerase association with nucleoprotein , but not polymerase assembly , is impaired in human cells during the course of infection .
	manualset3
257562	3	424033	15	NULL	NULL	NULL	NULL	nucleoprotein	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Avian Influenza A virus polymerase association with nucleoprotein , but not polymerase assembly , is impaired in human cells during the course of infection .
	manualset3
257563	4	424033	15	NULL	NULL	NULL	NULL	polymerase assembly	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Avian Influenza A virus polymerase association with nucleoprotein , but not polymerase assembly , is impaired in human cells during the course of infection .
	manualset3
257565	5	424033	15	NULL	NULL	NULL	NULL	human cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Avian Influenza A virus polymerase association with nucleoprotein , but not polymerase assembly , is impaired in human cells during the course of infection .
	manualset3
257566	6	424033	15	NULL	NULL	NULL	NULL	course of infection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Avian Influenza A virus polymerase association with nucleoprotein , but not polymerase assembly , is impaired in human cells during the course of infection .
	manualset3
257567	1	424034	15	NULL	NULL	NULL	NULL	Avoidance	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Avoidance and ICSS behavioral models dissociate TL-99 and 3-PPP from dopamine receptor antagonists .
	manualset3
257568	2	424034	15	NULL	NULL	NULL	NULL	ICSS behavioral models	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Avoidance and ICSS behavioral models dissociate TL-99 and 3-PPP from dopamine receptor antagonists .
	manualset3
257569	3	424034	15	NULL	NULL	NULL	NULL	TL-99	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Avoidance and ICSS behavioral models dissociate TL-99 and 3-PPP from dopamine receptor antagonists .
	manualset3
257570	4	424034	15	NULL	NULL	NULL	NULL	3-PPP 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Avoidance and ICSS behavioral models dissociate TL-99 and 3-PPP from dopamine receptor antagonists .
	manualset3
257571	5	424034	15	NULL	NULL	NULL	NULL	dopamine receptor antagonists	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Avoidance and ICSS behavioral models dissociate TL-99 and 3-PPP from dopamine receptor antagonists .
	manualset3
257572	1	424035	15	NULL	NULL	NULL	NULL	Avoidance	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Avoidance and hyperarousal in response to reminders of socially stressful events were common among patients ; more than one-third would have met criteria for PTSD if these events satisfied DSM-IV PTSD Criterion A. Frequency of this PTSD-like symptom pattern did not differ among patients who did and did not experience another event that did satisfy PTSD Criterion A. Implications of these findings for the treatment of social anxiety disorder are discussed .
	manualset3
257573	2	424035	15	NULL	NULL	NULL	NULL	hyperarousal	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Avoidance and hyperarousal in response to reminders of socially stressful events were common among patients ; more than one-third would have met criteria for PTSD if these events satisfied DSM-IV PTSD Criterion A. Frequency of this PTSD-like symptom pattern did not differ among patients who did and did not experience another event that did satisfy PTSD Criterion A. Implications of these findings for the treatment of social anxiety disorder are discussed .
	manualset3
257574	3	424035	15	NULL	NULL	NULL	NULL	response	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Avoidance and hyperarousal in response to reminders of socially stressful events were common among patients ; more than one-third would have met criteria for PTSD if these events satisfied DSM-IV PTSD Criterion A. Frequency of this PTSD-like symptom pattern did not differ among patients who did and did not experience another event that did satisfy PTSD Criterion A. Implications of these findings for the treatment of social anxiety disorder are discussed .
	manualset3
257575	4	424035	15	NULL	NULL	NULL	NULL	reminders of socially stressful events	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Avoidance and hyperarousal in response to reminders of socially stressful events were common among patients ; more than one-third would have met criteria for PTSD if these events satisfied DSM-IV PTSD Criterion A. Frequency of this PTSD-like symptom pattern did not differ among patients who did and did not experience another event that did satisfy PTSD Criterion A. Implications of these findings for the treatment of social anxiety disorder are discussed .
	manualset3
257576	5	424035	15	NULL	NULL	NULL	NULL	patients 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Avoidance and hyperarousal in response to reminders of socially stressful events were common among patients ; more than one-third would have met criteria for PTSD if these events satisfied DSM-IV PTSD Criterion A. Frequency of this PTSD-like symptom pattern did not differ among patients who did and did not experience another event that did satisfy PTSD Criterion A. Implications of these findings for the treatment of social anxiety disorder are discussed .
	manualset3
257577	6	424035	15	NULL	NULL	NULL	NULL	one-third	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Avoidance and hyperarousal in response to reminders of socially stressful events were common among patients ; more than one-third would have met criteria for PTSD if these events satisfied DSM-IV PTSD Criterion A. Frequency of this PTSD-like symptom pattern did not differ among patients who did and did not experience another event that did satisfy PTSD Criterion A. Implications of these findings for the treatment of social anxiety disorder are discussed .
	manualset3
257578	7	424035	15	NULL	NULL	NULL	NULL	criteria for PTSD	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Avoidance and hyperarousal in response to reminders of socially stressful events were common among patients ; more than one-third would have met criteria for PTSD if these events satisfied DSM-IV PTSD Criterion A. Frequency of this PTSD-like symptom pattern did not differ among patients who did and did not experience another event that did satisfy PTSD Criterion A. Implications of these findings for the treatment of social anxiety disorder are discussed .
	manualset3
257579	8	424035	15	NULL	NULL	NULL	NULL	events 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Avoidance and hyperarousal in response to reminders of socially stressful events were common among patients ; more than one-third would have met criteria for PTSD if these events satisfied DSM-IV PTSD Criterion A. Frequency of this PTSD-like symptom pattern did not differ among patients who did and did not experience another event that did satisfy PTSD Criterion A. Implications of these findings for the treatment of social anxiety disorder are discussed .
	manualset3
257590	9	424035	15	NULL	NULL	NULL	NULL	DSM-IV PTSD Criterion A	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Avoidance and hyperarousal in response to reminders of socially stressful events were common among patients ; more than one-third would have met criteria for PTSD if these events satisfied DSM-IV PTSD Criterion A. Frequency of this PTSD-like symptom pattern did not differ among patients who did and did not experience another event that did satisfy PTSD Criterion A. Implications of these findings for the treatment of social anxiety disorder are discussed .
	manualset3
257591	10	424035	15	NULL	NULL	NULL	NULL	Frequency	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Avoidance and hyperarousal in response to reminders of socially stressful events were common among patients ; more than one-third would have met criteria for PTSD if these events satisfied DSM-IV PTSD Criterion A. Frequency of this PTSD-like symptom pattern did not differ among patients who did and did not experience another event that did satisfy PTSD Criterion A. Implications of these findings for the treatment of social anxiety disorder are discussed .
	manualset3
257593	11	424035	15	NULL	NULL	NULL	NULL	PTSD-like symptom pattern	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Avoidance and hyperarousal in response to reminders of socially stressful events were common among patients ; more than one-third would have met criteria for PTSD if these events satisfied DSM-IV PTSD Criterion A. Frequency of this PTSD-like symptom pattern did not differ among patients who did and did not experience another event that did satisfy PTSD Criterion A. Implications of these findings for the treatment of social anxiety disorder are discussed .
	manualset3
257599	12	424035	15	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Avoidance and hyperarousal in response to reminders of socially stressful events were common among patients ; more than one-third would have met criteria for PTSD if these events satisfied DSM-IV PTSD Criterion A. Frequency of this PTSD-like symptom pattern did not differ among patients who did and did not experience another event that did satisfy PTSD Criterion A. Implications of these findings for the treatment of social anxiety disorder are discussed .
	manualset3
257604	13	424035	15	NULL	NULL	NULL	NULL	event	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Avoidance and hyperarousal in response to reminders of socially stressful events were common among patients ; more than one-third would have met criteria for PTSD if these events satisfied DSM-IV PTSD Criterion A. Frequency of this PTSD-like symptom pattern did not differ among patients who did and did not experience another event that did satisfy PTSD Criterion A. Implications of these findings for the treatment of social anxiety disorder are discussed .
	manualset3
257605	14	424035	15	NULL	NULL	NULL	NULL	PTSD Criterion A	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Avoidance and hyperarousal in response to reminders of socially stressful events were common among patients ; more than one-third would have met criteria for PTSD if these events satisfied DSM-IV PTSD Criterion A. Frequency of this PTSD-like symptom pattern did not differ among patients who did and did not experience another event that did satisfy PTSD Criterion A. Implications of these findings for the treatment of social anxiety disorder are discussed .
	manualset3
257606	15	424035	15	NULL	NULL	NULL	NULL	Implications 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Avoidance and hyperarousal in response to reminders of socially stressful events were common among patients ; more than one-third would have met criteria for PTSD if these events satisfied DSM-IV PTSD Criterion A. Frequency of this PTSD-like symptom pattern did not differ among patients who did and did not experience another event that did satisfy PTSD Criterion A. Implications of these findings for the treatment of social anxiety disorder are discussed .
	manualset3
257607	16	424035	15	NULL	NULL	NULL	NULL	treatment of social anxiety disorder	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Avoidance and hyperarousal in response to reminders of socially stressful events were common among patients ; more than one-third would have met criteria for PTSD if these events satisfied DSM-IV PTSD Criterion A. Frequency of this PTSD-like symptom pattern did not differ among patients who did and did not experience another event that did satisfy PTSD Criterion A. Implications of these findings for the treatment of social anxiety disorder are discussed .
	manualset3
257658	1	424036	15	NULL	NULL	NULL	NULL	Evaluation	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Evaluation of cerebrovascular reserve by xenon computed tomography in patients with ischemic stroke ) .
	manualset3
257661	2	424036	15	NULL	NULL	NULL	NULL	cerebrovascular reserve	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Evaluation of cerebrovascular reserve by xenon computed tomography in patients with ischemic stroke ) .
	manualset3
257663	3	424036	15	NULL	NULL	NULL	NULL	xenon computed tomography	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Evaluation of cerebrovascular reserve by xenon computed tomography in patients with ischemic stroke ) .
	manualset3
257664	4	424036	15	NULL	NULL	NULL	NULL	 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Evaluation of cerebrovascular reserve by xenon computed tomography in patients with ischemic stroke ) .
	manualset3
257665	5	424036	15	NULL	NULL	NULL	NULL	ischemic stroke	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Evaluation of cerebrovascular reserve by xenon computed tomography in patients with ischemic stroke ) .
	manualset3
257669	1	424037	15	NULL	NULL	NULL	NULL	asthma triggers	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Avoiding asthma triggers : a primer for patients .
	manualset3
257691	2	424037	15	NULL	NULL	NULL	NULL	primer	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Avoiding asthma triggers : a primer for patients .
	manualset3
257695	3	424037	15	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Avoiding asthma triggers : a primer for patients .
	manualset3
257705	1	424038	15	NULL	NULL	NULL	NULL	Awareness	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Awareness of diagnostic and clinical features of fibromyalgia among family physicians .
	manualset3
257707	2	424038	15	NULL	NULL	NULL	NULL	diagnostic features	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Awareness of diagnostic and clinical features of fibromyalgia among family physicians .
	manualset3
257708	3	424038	15	NULL	NULL	NULL	NULL	clinical features	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Awareness of diagnostic and clinical features of fibromyalgia among family physicians .
	manualset3
257709	4	424038	15	NULL	NULL	NULL	NULL	fibromyalgia 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Awareness of diagnostic and clinical features of fibromyalgia among family physicians .
	manualset3
257710	5	424038	15	NULL	NULL	NULL	NULL	family physicians 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Awareness of diagnostic and clinical features of fibromyalgia among family physicians .
	manualset3
257711	1	424039	15	NULL	NULL	NULL	NULL	Awareness	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Awareness of intermittent calf compressor injury in elderly people .
	manualset3
257712	2	424039	15	NULL	NULL	NULL	NULL	intermittent calf compressor injury	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Awareness of intermittent calf compressor injury in elderly people .
	manualset3
257713	3	424039	15	NULL	NULL	NULL	NULL	elderly people	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Awareness of intermittent calf compressor injury in elderly people .
	manualset3
257714	1	424040	15	NULL	NULL	NULL	NULL	Awareness	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Awareness of the above described features and familiarity with the clinical presentation of APNPRs is the best way to avoid a misdiagnosis .
	manualset3
257716	2	424040	15	NULL	NULL	NULL	NULL	features	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Awareness of the above described features and familiarity with the clinical presentation of APNPRs is the best way to avoid a misdiagnosis .
	manualset3
257717	3	424040	15	NULL	NULL	NULL	NULL	familiarity	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Awareness of the above described features and familiarity with the clinical presentation of APNPRs is the best way to avoid a misdiagnosis .
	manualset3
257718	4	424040	15	NULL	NULL	NULL	NULL	clinical presentation of APNPRs 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Awareness of the above described features and familiarity with the clinical presentation of APNPRs is the best way to avoid a misdiagnosis .
	manualset3
257719	5	424040	15	NULL	NULL	NULL	NULL	way	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Awareness of the above described features and familiarity with the clinical presentation of APNPRs is the best way to avoid a misdiagnosis .
	manualset3
257722	6	424040	15	NULL	NULL	NULL	NULL	misdiagnosis	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Awareness of the above described features and familiarity with the clinical presentation of APNPRs is the best way to avoid a misdiagnosis .
	manualset3
257723	1	424041	15	NULL	NULL	NULL	NULL	Awnt-1 / -5 A RNAs 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Awnt-1 / -5 A RNAs are stable until MBT then degraded before gastrulation .
	manualset3
257724	2	424041	15	NULL	NULL	NULL	NULL	MBT	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Awnt-1 / -5 A RNAs are stable until MBT then degraded before gastrulation .
	manualset3
257725	3	424041	15	NULL	NULL	NULL	NULL	gastrulation 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Awnt-1 / -5 A RNAs are stable until MBT then degraded before gastrulation .
	manualset3
257726	1	424042	15	NULL	NULL	NULL	NULL	Axillary hyperhydrosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Axillary hyperhydrosis in children and teenagers may be severe enough to affect social development .
	manualset3
257727	2	424042	15	NULL	NULL	NULL	NULL	children 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Axillary hyperhydrosis in children and teenagers may be severe enough to affect social development .
	manualset3
257728	3	424042	15	NULL	NULL	NULL	NULL	teenagers	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Axillary hyperhydrosis in children and teenagers may be severe enough to affect social development .
	manualset3
257729	4	424042	15	NULL	NULL	NULL	NULL	 social development	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Axillary hyperhydrosis in children and teenagers may be severe enough to affect social development .
	manualset3
257730	1	424043	15	NULL	NULL	NULL	NULL	Azelastine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Azelastine , a new generation antihistaminic , possesses certain antibacterial activity and is capable of inducing alteration in the bacterial membrane permeability .
	manualset3
257731	2	424043	15	NULL	NULL	NULL	NULL	new generation antihistaminic 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Azelastine , a new generation antihistaminic , possesses certain antibacterial activity and is capable of inducing alteration in the bacterial membrane permeability .
	manualset3
257732	3	424043	15	NULL	NULL	NULL	NULL	antibacterial activity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Azelastine , a new generation antihistaminic , possesses certain antibacterial activity and is capable of inducing alteration in the bacterial membrane permeability .
	manualset3
257733	4	424043	15	NULL	NULL	NULL	NULL	alteration	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Azelastine , a new generation antihistaminic , possesses certain antibacterial activity and is capable of inducing alteration in the bacterial membrane permeability .
	manualset3
257734	5	424043	15	NULL	NULL	NULL	NULL	bacterial membrane permeability	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Azelastine , a new generation antihistaminic , possesses certain antibacterial activity and is capable of inducing alteration in the bacterial membrane permeability .
	manualset3
257735	1	424044	15	NULL	NULL	NULL	NULL	Azelastine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Azelastine had no effect on the content of cyclic AMP or cyclic GMP .
	manualset3
257736	2	424044	15	NULL	NULL	NULL	NULL	effect	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Azelastine had no effect on the content of cyclic AMP or cyclic GMP .
	manualset3
257737	3	424044	15	NULL	NULL	NULL	NULL	content 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Azelastine had no effect on the content of cyclic AMP or cyclic GMP .
	manualset3
257738	4	424044	15	NULL	NULL	NULL	NULL	cyclic AMP	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Azelastine had no effect on the content of cyclic AMP or cyclic GMP .
	manualset3
257739	5	424044	15	NULL	NULL	NULL	NULL	cyclic GMP	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Azelastine had no effect on the content of cyclic AMP or cyclic GMP .
	manualset3
257740	1	424045	15	NULL	NULL	NULL	NULL	Azidohomoalanine	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Azidohomoalanine : a conformationally sensitive IR probe of protein folding , protein structure , and electrostatics .
	manualset3
257741	2	424045	15	NULL	NULL	NULL	NULL	conformationally sensitive IR probe	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Azidohomoalanine : a conformationally sensitive IR probe of protein folding , protein structure , and electrostatics .
	manualset3
257742	3	424045	15	NULL	NULL	NULL	NULL	protein folding	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Azidohomoalanine : a conformationally sensitive IR probe of protein folding , protein structure , and electrostatics .
	manualset3
257743	4	424045	15	NULL	NULL	NULL	NULL	protein structure	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Azidohomoalanine : a conformationally sensitive IR probe of protein folding , protein structure , and electrostatics .
	manualset3
257744	5	424045	15	NULL	NULL	NULL	NULL	electrostatics	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Azidohomoalanine : a conformationally sensitive IR probe of protein folding , protein structure , and electrostatics .
	manualset3
257745	1	424046	15	NULL	NULL	NULL	NULL	B-1008 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B-1008 is a water-soluble basic substance containing the spermidine moiety and possessing antibacterial activity against a wide range of bacterial species .
	manualset3
257746	2	424046	15	NULL	NULL	NULL	NULL	basic substance	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B-1008 is a water-soluble basic substance containing the spermidine moiety and possessing antibacterial activity against a wide range of bacterial species .
	manualset3
257747	3	424046	15	NULL	NULL	NULL	NULL	spermidine moiety	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B-1008 is a water-soluble basic substance containing the spermidine moiety and possessing antibacterial activity against a wide range of bacterial species .
	manualset3
257749	4	424046	15	NULL	NULL	NULL	NULL	antibacterial activity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B-1008 is a water-soluble basic substance containing the spermidine moiety and possessing antibacterial activity against a wide range of bacterial species .
	manualset3
257750	5	424046	15	NULL	NULL	NULL	NULL	wide range	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B-1008 is a water-soluble basic substance containing the spermidine moiety and possessing antibacterial activity against a wide range of bacterial species .
	manualset3
257752	6	424046	15	NULL	NULL	NULL	NULL	bacterial species	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B-1008 is a water-soluble basic substance containing the spermidine moiety and possessing antibacterial activity against a wide range of bacterial species .
	manualset3
257753	1	424047	15	NULL	NULL	NULL	NULL	Evaluation 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Evaluation of impact on health -- a central responsibility of the public health service ) .
	manualset3
257754	2	424047	15	NULL	NULL	NULL	NULL	impact on health	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Evaluation of impact on health -- a central responsibility of the public health service ) .
	manualset3
257755	3	424047	15	NULL	NULL	NULL	NULL	central responsibility	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Evaluation of impact on health -- a central responsibility of the public health service ) .
	manualset3
257756	4	424047	15	NULL	NULL	NULL	NULL	public health service	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Evaluation of impact on health -- a central responsibility of the public health service ) .
	manualset3
257764	1	424048	15	NULL	NULL	NULL	NULL	B-cell responses 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B-cell responses to vaccination at the extremes of age .
	manualset3
257766	2	424048	15	NULL	NULL	NULL	NULL	vaccination	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B-cell responses to vaccination at the extremes of age .
	manualset3
257775	3	424048	15	NULL	NULL	NULL	NULL	extremes of age 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B-cell responses to vaccination at the extremes of age .
	manualset3
257769	1	424049	15	NULL	NULL	NULL	NULL	B ( 1 ) homogeneity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B ( 1 ) homogeneity is intrinsically included via use of coil sensitivities in calculations .
	manualset3
257772	2	424049	15	NULL	NULL	NULL	NULL	use 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B ( 1 ) homogeneity is intrinsically included via use of coil sensitivities in calculations .
	manualset3
257776	3	424049	15	NULL	NULL	NULL	NULL	coil sensitivities	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B ( 1 ) homogeneity is intrinsically included via use of coil sensitivities in calculations .
	manualset3
257777	4	424049	15	NULL	NULL	NULL	NULL	calculations 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B ( 1 ) homogeneity is intrinsically included via use of coil sensitivities in calculations .
	manualset3
257784	1	424050	15	NULL	NULL	NULL	NULL	B ( a ) P	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B ( a ) P was the only compound to induce expression of aryl hydrocarbon receptor ( AhR ) - regulated genes , such as CYP1A1 and CYP1B1 , but did not induce cytokine/chemokine responses in BEAS-2B cells .
	manualset3
257785	2	424050	15	NULL	NULL	NULL	NULL	compound 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B ( a ) P was the only compound to induce expression of aryl hydrocarbon receptor ( AhR ) - regulated genes , such as CYP1A1 and CYP1B1 , but did not induce cytokine/chemokine responses in BEAS-2B cells .
	manualset3
257788	3	424050	15	NULL	NULL	NULL	NULL	expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B ( a ) P was the only compound to induce expression of aryl hydrocarbon receptor ( AhR ) - regulated genes , such as CYP1A1 and CYP1B1 , but did not induce cytokine/chemokine responses in BEAS-2B cells .
	manualset3
257790	4	424050	15	NULL	NULL	NULL	NULL	aryl hydrocarbon receptor ( AhR ) - regulated genes 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B ( a ) P was the only compound to induce expression of aryl hydrocarbon receptor ( AhR ) - regulated genes , such as CYP1A1 and CYP1B1 , but did not induce cytokine/chemokine responses in BEAS-2B cells .
	manualset3
257793	5	424050	15	NULL	NULL	NULL	NULL	CYP1A1 	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B ( a ) P was the only compound to induce expression of aryl hydrocarbon receptor ( AhR ) - regulated genes , such as CYP1A1 and CYP1B1 , but did not induce cytokine/chemokine responses in BEAS-2B cells .
	manualset3
257795	6	424050	15	NULL	NULL	NULL	NULL	CYP1B1	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B ( a ) P was the only compound to induce expression of aryl hydrocarbon receptor ( AhR ) - regulated genes , such as CYP1A1 and CYP1B1 , but did not induce cytokine/chemokine responses in BEAS-2B cells .
	manualset3
257796	7	424050	15	NULL	NULL	NULL	NULL	cytokine/chemokine responses	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B ( a ) P was the only compound to induce expression of aryl hydrocarbon receptor ( AhR ) - regulated genes , such as CYP1A1 and CYP1B1 , but did not induce cytokine/chemokine responses in BEAS-2B cells .
	manualset3
257797	8	424050	15	NULL	NULL	NULL	NULL	BEAS-2B cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B ( a ) P was the only compound to induce expression of aryl hydrocarbon receptor ( AhR ) - regulated genes , such as CYP1A1 and CYP1B1 , but did not induce cytokine/chemokine responses in BEAS-2B cells .
	manualset3
257798	1	424051	15	NULL	NULL	NULL	NULL	B cell chemotaxis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B cell chemotaxis occurs in response to specific chemokine gradients and is critical for homeostasis and immune response .
	manualset3
257799	2	424051	15	NULL	NULL	NULL	NULL	response 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B cell chemotaxis occurs in response to specific chemokine gradients and is critical for homeostasis and immune response .
	manualset3
257800	3	424051	15	NULL	NULL	NULL	NULL	chemokine gradients	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B cell chemotaxis occurs in response to specific chemokine gradients and is critical for homeostasis and immune response .
	manualset3
257801	4	424051	15	NULL	NULL	NULL	NULL	homeostasis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B cell chemotaxis occurs in response to specific chemokine gradients and is critical for homeostasis and immune response .
	manualset3
257802	5	424051	15	NULL	NULL	NULL	NULL	immune response	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B cell chemotaxis occurs in response to specific chemokine gradients and is critical for homeostasis and immune response .
	manualset3
257809	1	424052	15	NULL	NULL	NULL	NULL	B sepsis LAT 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B sepsis LAT was positive , the test was performed 2.5 h-19 h after onset of RDS .
	manualset3
257811	2	424052	15	NULL	NULL	NULL	NULL	test 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B sepsis LAT was positive , the test was performed 2.5 h-19 h after onset of RDS .
	manualset3
257813	3	424052	15	NULL	NULL	NULL	NULL	2.5 h-19 h	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B sepsis LAT was positive , the test was performed 2.5 h-19 h after onset of RDS .
	manualset3
257816	4	424052	15	NULL	NULL	NULL	NULL	onset of RDS	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B sepsis LAT was positive , the test was performed 2.5 h-19 h after onset of RDS .
	manualset3
257818	1	424053	15	NULL	NULL	NULL	NULL	B	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B was probably via formation of complexes with membrane components .
	manualset3
257819	2	424053	15	NULL	NULL	NULL	NULL	formation of complexes	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B was probably via formation of complexes with membrane components .
	manualset3
257822	3	424053	15	NULL	NULL	NULL	NULL	membrane components	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B was probably via formation of complexes with membrane components .
	manualset3
257830	1	424054	15	NULL	NULL	NULL	NULL	B700	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B700 , a murine melanoma-specific antigen , is a member of the serum albumin protein family .
	manualset3
259827	2	424054	15	NULL	NULL	NULL	NULL	murine melanoma-specific antigen	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B700 , a murine melanoma-specific antigen , is a member of the serum albumin protein family .
	manualset3
259833	3	424054	15	NULL	NULL	NULL	NULL	member	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B700 , a murine melanoma-specific antigen , is a member of the serum albumin protein family .
	manualset3
259834	4	424054	15	NULL	NULL	NULL	NULL	serum albumin protein family	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	B700 , a murine melanoma-specific antigen , is a member of the serum albumin protein family .
	manualset3
259838	1	424055	15	NULL	NULL	NULL	NULL	BACKGROUND	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BACKGROUND : Pleural sarcoidosis is not a rare disease , and some patients with sarcoidosis experience chest pain , although the cause is often unknown .
	manualset3
259841	2	424055	15	NULL	NULL	NULL	NULL	Pleural sarcoidosis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BACKGROUND : Pleural sarcoidosis is not a rare disease , and some patients with sarcoidosis experience chest pain , although the cause is often unknown .
	manualset3
259842	3	424055	15	NULL	NULL	NULL	NULL	disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BACKGROUND : Pleural sarcoidosis is not a rare disease , and some patients with sarcoidosis experience chest pain , although the cause is often unknown .
	manualset3
259843	4	424055	15	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BACKGROUND : Pleural sarcoidosis is not a rare disease , and some patients with sarcoidosis experience chest pain , although the cause is often unknown .
	manualset3
259844	5	424055	15	NULL	NULL	NULL	NULL	sarcoidosis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BACKGROUND : Pleural sarcoidosis is not a rare disease , and some patients with sarcoidosis experience chest pain , although the cause is often unknown .
	manualset3
259845	6	424055	15	NULL	NULL	NULL	NULL	chest pain	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BACKGROUND : Pleural sarcoidosis is not a rare disease , and some patients with sarcoidosis experience chest pain , although the cause is often unknown .
	manualset3
259847	7	424055	15	NULL	NULL	NULL	NULL	cause	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BACKGROUND : Pleural sarcoidosis is not a rare disease , and some patients with sarcoidosis experience chest pain , although the cause is often unknown .
	manualset3
259851	1	424056	15	NULL	NULL	NULL	NULL	Examination 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Examination of the blood in morbus caeruleus .
	manualset3
259853	2	424056	15	NULL	NULL	NULL	NULL	blood 	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Examination of the blood in morbus caeruleus .
	manualset3
259854	3	424056	15	NULL	NULL	NULL	NULL	morbus caeruleus	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Examination of the blood in morbus caeruleus .
	manualset3
259859	1	424057	15	NULL	NULL	NULL	NULL	BACKGROUND	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BACKGROUND AND PURPOSE The potent pro-angiogenic growth factors VEGF-A and basic fibroblast growth factor ( bFGF ) exert their effects by binding VEGF receptor 2 and FGF receptor tyrosine kinases , respectively .
	manualset3
259860	2	424057	15	NULL	NULL	NULL	NULL	PURPOSE	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BACKGROUND AND PURPOSE The potent pro-angiogenic growth factors VEGF-A and basic fibroblast growth factor ( bFGF ) exert their effects by binding VEGF receptor 2 and FGF receptor tyrosine kinases , respectively .
	manualset3
259861	3	424057	15	NULL	NULL	NULL	NULL	pro-angiogenic growth factor VEGF-A	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BACKGROUND AND PURPOSE The potent pro-angiogenic growth factors VEGF-A and basic fibroblast growth factor ( bFGF ) exert their effects by binding VEGF receptor 2 and FGF receptor tyrosine kinases , respectively .
	manualset3
259862	4	424057	15	NULL	NULL	NULL	NULL	basic fibroblast growth factor ( bFGF )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BACKGROUND AND PURPOSE The potent pro-angiogenic growth factors VEGF-A and basic fibroblast growth factor ( bFGF ) exert their effects by binding VEGF receptor 2 and FGF receptor tyrosine kinases , respectively .
	manualset3
259863	5	424057	15	NULL	NULL	NULL	NULL	effects	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BACKGROUND AND PURPOSE The potent pro-angiogenic growth factors VEGF-A and basic fibroblast growth factor ( bFGF ) exert their effects by binding VEGF receptor 2 and FGF receptor tyrosine kinases , respectively .
	manualset3
259864	6	424057	15	NULL	NULL	NULL	NULL	binding VEGF receptor 2	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BACKGROUND AND PURPOSE The potent pro-angiogenic growth factors VEGF-A and basic fibroblast growth factor ( bFGF ) exert their effects by binding VEGF receptor 2 and FGF receptor tyrosine kinases , respectively .
	manualset3
259865	7	424057	15	NULL	NULL	NULL	NULL	binding FGF receptor tyrosine kinases	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BACKGROUND AND PURPOSE The potent pro-angiogenic growth factors VEGF-A and basic fibroblast growth factor ( bFGF ) exert their effects by binding VEGF receptor 2 and FGF receptor tyrosine kinases , respectively .
	manualset3
259866	1	424058	15	NULL	NULL	NULL	NULL	BALB/c mice	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BALB/c mice were infected orally with Salmonella dublin strains Lane and LD842 , an isogenic derivative of the former that is avirulent because it was cured of its 80-kilobase-pair virulence plasmid pSDL2 .
	manualset3
259867	2	424058	15	NULL	NULL	NULL	NULL	Salmonella dublin strain Lane	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BALB/c mice were infected orally with Salmonella dublin strains Lane and LD842 , an isogenic derivative of the former that is avirulent because it was cured of its 80-kilobase-pair virulence plasmid pSDL2 .
	manualset3
259868	3	424058	15	NULL	NULL	NULL	NULL	Salmonella dublin strain LD842 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BALB/c mice were infected orally with Salmonella dublin strains Lane and LD842 , an isogenic derivative of the former that is avirulent because it was cured of its 80-kilobase-pair virulence plasmid pSDL2 .
	manualset3
259869	4	424058	15	NULL	NULL	NULL	NULL	80-kilobase-pair virulence plasmid pSDL2	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BALB/c mice were infected orally with Salmonella dublin strains Lane and LD842 , an isogenic derivative of the former that is avirulent because it was cured of its 80-kilobase-pair virulence plasmid pSDL2 .
	manualset3
259870	1	424059	15	NULL	NULL	NULL	NULL	BCE	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BCE added either with NMDA ( 1 mM ) or 1 h later had lesser , but still significant , protective actions .
	manualset3
259871	2	424059	15	NULL	NULL	NULL	NULL	NMDA ( 1 mM )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BCE added either with NMDA ( 1 mM ) or 1 h later had lesser , but still significant , protective actions .
	manualset3
259872	3	424059	15	NULL	NULL	NULL	NULL	1 h later	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BCE added either with NMDA ( 1 mM ) or 1 h later had lesser , but still significant , protective actions .
	manualset3
259873	4	424059	15	NULL	NULL	NULL	NULL	significant actions 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BCE added either with NMDA ( 1 mM ) or 1 h later had lesser , but still significant , protective actions .
	manualset3
259874	5	424059	15	NULL	NULL	NULL	NULL	protective actions 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BCE added either with NMDA ( 1 mM ) or 1 h later had lesser , but still significant , protective actions .
	manualset3
259875	1	424060	15	NULL	NULL	NULL	NULL	BH4	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BH4 exhibited a range of potency comparable to that of 6-hydroxydopamine .
	manualset3
259876	2	424060	15	NULL	NULL	NULL	NULL	range of potency	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BH4 exhibited a range of potency comparable to that of 6-hydroxydopamine .
	manualset3
259877	3	424060	15	NULL	NULL	NULL	NULL	6-hydroxydopamine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BH4 exhibited a range of potency comparable to that of 6-hydroxydopamine .
	manualset3
260709	1	424061	15	NULL	NULL	NULL	NULL	BII anastomosis	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BII anastomosis was followed by a significantly lower rate of H. pylori infection ( 17/37 ; 45.9 % ) than BI anastomosis ( 51/72 ; 70.8 % ; p = 0.01 ) according to the results of PCR .
	manualset3
260710	2	424061	15	NULL	NULL	NULL	NULL	rate 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BII anastomosis was followed by a significantly lower rate of H. pylori infection ( 17/37 ; 45.9 % ) than BI anastomosis ( 51/72 ; 70.8 % ; p = 0.01 ) according to the results of PCR .
	manualset3
260711	3	424061	15	NULL	NULL	NULL	NULL	H. pylori infection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BII anastomosis was followed by a significantly lower rate of H. pylori infection ( 17/37 ; 45.9 % ) than BI anastomosis ( 51/72 ; 70.8 % ; p = 0.01 ) according to the results of PCR .
	manualset3
260712	4	424061	15	NULL	NULL	NULL	NULL	 17/37 ; 45.9 %	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BII anastomosis was followed by a significantly lower rate of H. pylori infection ( 17/37 ; 45.9 % ) than BI anastomosis ( 51/72 ; 70.8 % ; p = 0.01 ) according to the results of PCR .
	manualset3
260713	5	424061	15	NULL	NULL	NULL	NULL	BI anastomosis 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BII anastomosis was followed by a significantly lower rate of H. pylori infection ( 17/37 ; 45.9 % ) than BI anastomosis ( 51/72 ; 70.8 % ; p = 0.01 ) according to the results of PCR .
	manualset3
260714	6	424061	15	NULL	NULL	NULL	NULL	51/72 ; 70.8 % ; p = 0.01	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BII anastomosis was followed by a significantly lower rate of H. pylori infection ( 17/37 ; 45.9 % ) than BI anastomosis ( 51/72 ; 70.8 % ; p = 0.01 ) according to the results of PCR .
	manualset3
260715	7	424061	15	NULL	NULL	NULL	NULL	results of PCR	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BII anastomosis was followed by a significantly lower rate of H. pylori infection ( 17/37 ; 45.9 % ) than BI anastomosis ( 51/72 ; 70.8 % ; p = 0.01 ) according to the results of PCR .
	manualset3
260716	1	424062	15	NULL	NULL	NULL	NULL	BK virus antibody	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BK virus antibody in population of various age groups in Beijing .
	manualset3
260719	2	424062	15	NULL	NULL	NULL	NULL	population	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BK virus antibody in population of various age groups in Beijing .
	manualset3
260721	3	424062	15	NULL	NULL	NULL	NULL	age groups	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BK virus antibody in population of various age groups in Beijing .
	manualset3
260722	4	424062	15	NULL	NULL	NULL	NULL	Beijing	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BK virus antibody in population of various age groups in Beijing .
	manualset3
260723	1	424063	15	NULL	NULL	NULL	NULL	Experience	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experience in the work of the nurse-anesthetist ) .
	manualset3
260724	2	424063	15	NULL	NULL	NULL	NULL	work	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experience in the work of the nurse-anesthetist ) .
	manualset3
260725	3	424063	15	NULL	NULL	NULL	NULL	nurse-anesthetist	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experience in the work of the nurse-anesthetist ) .
	manualset3
260726	1	424064	15	NULL	NULL	NULL	NULL	BK virus nephropathy	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BK virus nephropathy is a common cause of graft loss in kidney transplant recipients .
	manualset3
260727	2	424064	15	NULL	NULL	NULL	NULL	cause of graft loss	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BK virus nephropathy is a common cause of graft loss in kidney transplant recipients .
	manualset3
260728	3	424064	15	NULL	NULL	NULL	NULL	kidney transplant recipients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BK virus nephropathy is a common cause of graft loss in kidney transplant recipients .
	manualset3
260731	1	424065	15	NULL	NULL	NULL	NULL	BLNK	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BLNK is a critical adaptor molecule for PLC-gamma2 tyrosine phosphorylation through its binding to the PLC-gamma2 SH2 domains .
	manualset3
260736	2	424065	15	NULL	NULL	NULL	NULL	adaptor molecule 	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BLNK is a critical adaptor molecule for PLC-gamma2 tyrosine phosphorylation through its binding to the PLC-gamma2 SH2 domains .
	manualset3
260738	3	424065	15	NULL	NULL	NULL	NULL	PLC-gamma2 tyrosine phosphorylation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BLNK is a critical adaptor molecule for PLC-gamma2 tyrosine phosphorylation through its binding to the PLC-gamma2 SH2 domains .
	manualset3
260742	4	424065	15	NULL	NULL	NULL	NULL	PLC-gamma2 SH2 domains	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BLNK is a critical adaptor molecule for PLC-gamma2 tyrosine phosphorylation through its binding to the PLC-gamma2 SH2 domains .
	manualset3
260743	1	424066	15	NULL	NULL	NULL	NULL	BM	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BM from 30 AA and 10 normal donors was then stained for CD34 , Fas-ag and 7-AminoActinomycin D. The proportion of CD34 ( + ) Fas ( + ) cells was higher in untreated AA ( P = 0.0001 ) than in normal donors .
	manualset3
260744	2	424066	15	NULL	NULL	NULL	NULL	30 AA	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BM from 30 AA and 10 normal donors was then stained for CD34 , Fas-ag and 7-AminoActinomycin D. The proportion of CD34 ( + ) Fas ( + ) cells was higher in untreated AA ( P = 0.0001 ) than in normal donors .
	manualset3
260745	3	424066	15	NULL	NULL	NULL	NULL	10 normal donors	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BM from 30 AA and 10 normal donors was then stained for CD34 , Fas-ag and 7-AminoActinomycin D. The proportion of CD34 ( + ) Fas ( + ) cells was higher in untreated AA ( P = 0.0001 ) than in normal donors .
	manualset3
260754	4	424066	15	NULL	NULL	NULL	NULL	CD34	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BM from 30 AA and 10 normal donors was then stained for CD34 , Fas-ag and 7-AminoActinomycin D. The proportion of CD34 ( + ) Fas ( + ) cells was higher in untreated AA ( P = 0.0001 ) than in normal donors .
	manualset3
260759	5	424066	15	NULL	NULL	NULL	NULL	Fas-ag 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BM from 30 AA and 10 normal donors was then stained for CD34 , Fas-ag and 7-AminoActinomycin D. The proportion of CD34 ( + ) Fas ( + ) cells was higher in untreated AA ( P = 0.0001 ) than in normal donors .
	manualset3
260762	6	424066	15	NULL	NULL	NULL	NULL	7-AminoActinomycin D	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BM from 30 AA and 10 normal donors was then stained for CD34 , Fas-ag and 7-AminoActinomycin D. The proportion of CD34 ( + ) Fas ( + ) cells was higher in untreated AA ( P = 0.0001 ) than in normal donors .
	manualset3
260763	7	424066	15	NULL	NULL	NULL	NULL	proportion 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BM from 30 AA and 10 normal donors was then stained for CD34 , Fas-ag and 7-AminoActinomycin D. The proportion of CD34 ( + ) Fas ( + ) cells was higher in untreated AA ( P = 0.0001 ) than in normal donors .
	manualset3
260765	8	424066	15	NULL	NULL	NULL	NULL	CD34 ( + ) Fas ( + ) cells 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BM from 30 AA and 10 normal donors was then stained for CD34 , Fas-ag and 7-AminoActinomycin D. The proportion of CD34 ( + ) Fas ( + ) cells was higher in untreated AA ( P = 0.0001 ) than in normal donors .
	manualset3
260766	9	424066	15	NULL	NULL	NULL	NULL	untreated AA 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BM from 30 AA and 10 normal donors was then stained for CD34 , Fas-ag and 7-AminoActinomycin D. The proportion of CD34 ( + ) Fas ( + ) cells was higher in untreated AA ( P = 0.0001 ) than in normal donors .
	manualset3
260767	10	424066	15	NULL	NULL	NULL	NULL	P = 0.0001	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BM from 30 AA and 10 normal donors was then stained for CD34 , Fas-ag and 7-AminoActinomycin D. The proportion of CD34 ( + ) Fas ( + ) cells was higher in untreated AA ( P = 0.0001 ) than in normal donors .
	manualset3
260768	11	424066	15	NULL	NULL	NULL	NULL	normal donors	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BM from 30 AA and 10 normal donors was then stained for CD34 , Fas-ag and 7-AminoActinomycin D. The proportion of CD34 ( + ) Fas ( + ) cells was higher in untreated AA ( P = 0.0001 ) than in normal donors .
	manualset3
260773	1	424067	15	NULL	NULL	NULL	NULL	BMP-2 signaling 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BMP-2 / BMP-RII signaling prevented PDGF-BB-induced proliferation of human and murine pulmonary artery SMCs ( PASMCs ) by decreasing nuclear phospho-ERK and inducing DNA binding of PPARgamma that is independent of Smad1/5/8 phosphorylation .
	manualset3
260774	2	424067	15	NULL	NULL	NULL	NULL	BMP-RII signaling 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BMP-2 / BMP-RII signaling prevented PDGF-BB-induced proliferation of human and murine pulmonary artery SMCs ( PASMCs ) by decreasing nuclear phospho-ERK and inducing DNA binding of PPARgamma that is independent of Smad1/5/8 phosphorylation .
	manualset3
260777	3	424067	15	NULL	NULL	NULL	NULL	PDGF-BB-induced proliferation 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BMP-2 / BMP-RII signaling prevented PDGF-BB-induced proliferation of human and murine pulmonary artery SMCs ( PASMCs ) by decreasing nuclear phospho-ERK and inducing DNA binding of PPARgamma that is independent of Smad1/5/8 phosphorylation .
	manualset3
260780	4	424067	15	NULL	NULL	NULL	NULL	human pulmonary artery SMCs ( PASMCs ) 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BMP-2 / BMP-RII signaling prevented PDGF-BB-induced proliferation of human and murine pulmonary artery SMCs ( PASMCs ) by decreasing nuclear phospho-ERK and inducing DNA binding of PPARgamma that is independent of Smad1/5/8 phosphorylation .
	manualset3
260781	5	424067	15	NULL	NULL	NULL	NULL	murine pulmonary artery SMCs ( PASMCs )	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BMP-2 / BMP-RII signaling prevented PDGF-BB-induced proliferation of human and murine pulmonary artery SMCs ( PASMCs ) by decreasing nuclear phospho-ERK and inducing DNA binding of PPARgamma that is independent of Smad1/5/8 phosphorylation .
	manualset3
260782	6	424067	15	NULL	NULL	NULL	NULL	decreasing nuclear phospho-ERK 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BMP-2 / BMP-RII signaling prevented PDGF-BB-induced proliferation of human and murine pulmonary artery SMCs ( PASMCs ) by decreasing nuclear phospho-ERK and inducing DNA binding of PPARgamma that is independent of Smad1/5/8 phosphorylation .
	manualset3
260783	7	424067	15	NULL	NULL	NULL	NULL	inducing DNA binding of PPARgamma	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BMP-2 / BMP-RII signaling prevented PDGF-BB-induced proliferation of human and murine pulmonary artery SMCs ( PASMCs ) by decreasing nuclear phospho-ERK and inducing DNA binding of PPARgamma that is independent of Smad1/5/8 phosphorylation .
	manualset3
260784	8	424067	15	NULL	NULL	NULL	NULL	Smad1/5/8 phosphorylation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BMP-2 / BMP-RII signaling prevented PDGF-BB-induced proliferation of human and murine pulmonary artery SMCs ( PASMCs ) by decreasing nuclear phospho-ERK and inducing DNA binding of PPARgamma that is independent of Smad1/5/8 phosphorylation .
	manualset3
260785	1	424068	15	NULL	NULL	NULL	NULL	BMP-2	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BMP-2 induces transcriptional activation of JunB expression as early as 30 min after ligand addition , reaching maximal levels after 90 min .
	manualset3
260786	2	424068	15	NULL	NULL	NULL	NULL	transcriptional activation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BMP-2 induces transcriptional activation of JunB expression as early as 30 min after ligand addition , reaching maximal levels after 90 min .
	manualset3
260787	3	424068	15	NULL	NULL	NULL	NULL	JunB expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BMP-2 induces transcriptional activation of JunB expression as early as 30 min after ligand addition , reaching maximal levels after 90 min .
	manualset3
260788	4	424068	15	NULL	NULL	NULL	NULL	30 min after ligand addition	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BMP-2 induces transcriptional activation of JunB expression as early as 30 min after ligand addition , reaching maximal levels after 90 min .
	manualset3
260789	5	424068	15	NULL	NULL	NULL	NULL	levels 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BMP-2 induces transcriptional activation of JunB expression as early as 30 min after ligand addition , reaching maximal levels after 90 min .
	manualset3
260790	6	424068	15	NULL	NULL	NULL	NULL	90 min	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BMP-2 induces transcriptional activation of JunB expression as early as 30 min after ligand addition , reaching maximal levels after 90 min .
	manualset3
260791	1	424069	15	NULL	NULL	NULL	NULL	BMP type II receptor deficiency	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BMP type II receptor deficiency confers resistance to growth inhibition by TGF - in pulmonary artery smooth muscle cells : role of proinflammatory cytokines .
	manualset3
260792	2	424069	15	NULL	NULL	NULL	NULL	resistance to growth inhibition 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BMP type II receptor deficiency confers resistance to growth inhibition by TGF - in pulmonary artery smooth muscle cells : role of proinflammatory cytokines .
	manualset3
260793	3	424069	15	NULL	NULL	NULL	NULL	TGF	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BMP type II receptor deficiency confers resistance to growth inhibition by TGF - in pulmonary artery smooth muscle cells : role of proinflammatory cytokines .
	manualset3
260794	4	424069	15	NULL	NULL	NULL	NULL	pulmonary artery smooth muscle cells 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BMP type II receptor deficiency confers resistance to growth inhibition by TGF - in pulmonary artery smooth muscle cells : role of proinflammatory cytokines .
	manualset3
260795	5	424069	15	NULL	NULL	NULL	NULL	role	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BMP type II receptor deficiency confers resistance to growth inhibition by TGF - in pulmonary artery smooth muscle cells : role of proinflammatory cytokines .
	manualset3
260796	6	424069	15	NULL	NULL	NULL	NULL	proinflammatory cytokines	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BMP type II receptor deficiency confers resistance to growth inhibition by TGF - in pulmonary artery smooth muscle cells : role of proinflammatory cytokines .
	manualset3
260797	1	424070	15	NULL	NULL	NULL	NULL	BODIPY-conantokin-G binding clusters 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BODIPY-conantokin-G binding clusters were associated with presynaptic nerve terminals while isolated BODIPY-conantokin-G binding sites were not always opposed to terminals .
	manualset3
260798	2	424070	15	NULL	NULL	NULL	NULL	presynaptic nerve terminals	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BODIPY-conantokin-G binding clusters were associated with presynaptic nerve terminals while isolated BODIPY-conantokin-G binding sites were not always opposed to terminals .
	manualset3
260799	3	424070	15	NULL	NULL	NULL	NULL	BODIPY-conantokin-G binding sites 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BODIPY-conantokin-G binding clusters were associated with presynaptic nerve terminals while isolated BODIPY-conantokin-G binding sites were not always opposed to terminals .
	manualset3
260800	4	424070	15	NULL	NULL	NULL	NULL	terminals	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BODIPY-conantokin-G binding clusters were associated with presynaptic nerve terminals while isolated BODIPY-conantokin-G binding sites were not always opposed to terminals .
	manualset3
260801	1	424071	15	NULL	NULL	NULL	NULL	BP reduction 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BP reduction was significantly greater with zofenopril ( 30 mg/day ) during the initial 4 weeks of treatment compared with enalapril ( 20 mg/day ) .
	manualset3
260802	2	424071	15	NULL	NULL	NULL	NULL	zofenopril	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BP reduction was significantly greater with zofenopril ( 30 mg/day ) during the initial 4 weeks of treatment compared with enalapril ( 20 mg/day ) .
	manualset3
260803	3	424071	15	NULL	NULL	NULL	NULL	30 mg/day	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BP reduction was significantly greater with zofenopril ( 30 mg/day ) during the initial 4 weeks of treatment compared with enalapril ( 20 mg/day ) .
	manualset3
260804	4	424071	15	NULL	NULL	NULL	NULL	initial 4 weeks of treatment 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BP reduction was significantly greater with zofenopril ( 30 mg/day ) during the initial 4 weeks of treatment compared with enalapril ( 20 mg/day ) .
	manualset3
260805	5	424071	15	NULL	NULL	NULL	NULL	enalapril 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BP reduction was significantly greater with zofenopril ( 30 mg/day ) during the initial 4 weeks of treatment compared with enalapril ( 20 mg/day ) .
	manualset3
260806	6	424071	15	NULL	NULL	NULL	NULL	20 mg/day	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BP reduction was significantly greater with zofenopril ( 30 mg/day ) during the initial 4 weeks of treatment compared with enalapril ( 20 mg/day ) .
	manualset3
260807	1	424072	15	NULL	NULL	NULL	NULL	BRACking news	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BRACking news on triple-negative/basal-like breast cancers : how BRCA1 deficiency may result in the development of a selective tumor subtype .
	manualset3
260808	2	424072	15	NULL	NULL	NULL	NULL	triple-negative breast cancers	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BRACking news on triple-negative/basal-like breast cancers : how BRCA1 deficiency may result in the development of a selective tumor subtype .
	manualset3
260809	3	424072	15	NULL	NULL	NULL	NULL	basal-like breast cancers	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BRACking news on triple-negative/basal-like breast cancers : how BRCA1 deficiency may result in the development of a selective tumor subtype .
	manualset3
260810	4	424072	15	NULL	NULL	NULL	NULL	BRCA1 deficiency	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BRACking news on triple-negative/basal-like breast cancers : how BRCA1 deficiency may result in the development of a selective tumor subtype .
	manualset3
260811	5	424072	15	NULL	NULL	NULL	NULL	development of a selective tumor subtype	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BRACking news on triple-negative/basal-like breast cancers : how BRCA1 deficiency may result in the development of a selective tumor subtype .
	manualset3
260812	1	424073	15	NULL	NULL	NULL	NULL	BSAP	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BSAP activated the promoter in transfected cells , and the BSAP site was occupied in a tissue-specific manner in vivo .
	manualset3
260815	2	424073	15	NULL	NULL	NULL	NULL	promoter	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BSAP activated the promoter in transfected cells , and the BSAP site was occupied in a tissue-specific manner in vivo .
	manualset3
260817	3	424073	15	NULL	NULL	NULL	NULL	transfected cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BSAP activated the promoter in transfected cells , and the BSAP site was occupied in a tissue-specific manner in vivo .
	manualset3
260820	4	424073	15	NULL	NULL	NULL	NULL	BSAP site	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BSAP activated the promoter in transfected cells , and the BSAP site was occupied in a tissue-specific manner in vivo .
	manualset3
260821	5	424073	15	NULL	NULL	NULL	NULL	tissue-specific manner 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BSAP activated the promoter in transfected cells , and the BSAP site was occupied in a tissue-specific manner in vivo .
	manualset3
260822	1	424074	15	NULL	NULL	NULL	NULL	BSM sensitivity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BSM sensitivity to ES , expressed as the log ES frequency producing 50 % of Tmax ( i.e. , log ES50 ) was also increased ( p less than 0.001 ) in the presence of CTZ as indicated by a fall in the mean + / - SEM log ES50 from 1.05 + / - 0.05 to 0.804 + / - 0.09 Hz .
	manualset3
260824	2	424074	15	NULL	NULL	NULL	NULL	ES	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BSM sensitivity to ES , expressed as the log ES frequency producing 50 % of Tmax ( i.e. , log ES50 ) was also increased ( p less than 0.001 ) in the presence of CTZ as indicated by a fall in the mean + / - SEM log ES50 from 1.05 + / - 0.05 to 0.804 + / - 0.09 Hz .
	manualset3
260826	3	424074	15	NULL	NULL	NULL	NULL	log ES frequency	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BSM sensitivity to ES , expressed as the log ES frequency producing 50 % of Tmax ( i.e. , log ES50 ) was also increased ( p less than 0.001 ) in the presence of CTZ as indicated by a fall in the mean + / - SEM log ES50 from 1.05 + / - 0.05 to 0.804 + / - 0.09 Hz .
	manualset3
260827	4	424074	15	NULL	NULL	NULL	NULL	50 % of Tmax	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BSM sensitivity to ES , expressed as the log ES frequency producing 50 % of Tmax ( i.e. , log ES50 ) was also increased ( p less than 0.001 ) in the presence of CTZ as indicated by a fall in the mean + / - SEM log ES50 from 1.05 + / - 0.05 to 0.804 + / - 0.09 Hz .
	manualset3
260828	5	424074	15	NULL	NULL	NULL	NULL	log ES50 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BSM sensitivity to ES , expressed as the log ES frequency producing 50 % of Tmax ( i.e. , log ES50 ) was also increased ( p less than 0.001 ) in the presence of CTZ as indicated by a fall in the mean + / - SEM log ES50 from 1.05 + / - 0.05 to 0.804 + / - 0.09 Hz .
	manualset3
260829	6	424074	15	NULL	NULL	NULL	NULL	p less than 0.001	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BSM sensitivity to ES , expressed as the log ES frequency producing 50 % of Tmax ( i.e. , log ES50 ) was also increased ( p less than 0.001 ) in the presence of CTZ as indicated by a fall in the mean + / - SEM log ES50 from 1.05 + / - 0.05 to 0.804 + / - 0.09 Hz .
	manualset3
260830	7	424074	15	NULL	NULL	NULL	NULL	presence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BSM sensitivity to ES , expressed as the log ES frequency producing 50 % of Tmax ( i.e. , log ES50 ) was also increased ( p less than 0.001 ) in the presence of CTZ as indicated by a fall in the mean + / - SEM log ES50 from 1.05 + / - 0.05 to 0.804 + / - 0.09 Hz .
	manualset3
260835	8	424074	15	NULL	NULL	NULL	NULL	CTZ 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BSM sensitivity to ES , expressed as the log ES frequency producing 50 % of Tmax ( i.e. , log ES50 ) was also increased ( p less than 0.001 ) in the presence of CTZ as indicated by a fall in the mean + / - SEM log ES50 from 1.05 + / - 0.05 to 0.804 + / - 0.09 Hz .
	manualset3
260836	9	424074	15	NULL	NULL	NULL	NULL	fall in the mean + / - SEM log ES50 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BSM sensitivity to ES , expressed as the log ES frequency producing 50 % of Tmax ( i.e. , log ES50 ) was also increased ( p less than 0.001 ) in the presence of CTZ as indicated by a fall in the mean + / - SEM log ES50 from 1.05 + / - 0.05 to 0.804 + / - 0.09 Hz .
	manualset3
260837	10	424074	15	NULL	NULL	NULL	NULL	1.05 + / - 0.05 Hz	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BSM sensitivity to ES , expressed as the log ES frequency producing 50 % of Tmax ( i.e. , log ES50 ) was also increased ( p less than 0.001 ) in the presence of CTZ as indicated by a fall in the mean + / - SEM log ES50 from 1.05 + / - 0.05 to 0.804 + / - 0.09 Hz .
	manualset3
260838	11	424074	15	NULL	NULL	NULL	NULL	0.804 + / - 0.09 Hz	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BSM sensitivity to ES , expressed as the log ES frequency producing 50 % of Tmax ( i.e. , log ES50 ) was also increased ( p less than 0.001 ) in the presence of CTZ as indicated by a fall in the mean + / - SEM log ES50 from 1.05 + / - 0.05 to 0.804 + / - 0.09 Hz .
	manualset3
260841	1	424075	15	NULL	NULL	NULL	NULL	Bacillary white diarrhoea	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacillary white diarrhoea of poultry and its eradication in the Union of South Africa .
	manualset3
260843	2	424075	15	NULL	NULL	NULL	NULL	poultry	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacillary white diarrhoea of poultry and its eradication in the Union of South Africa .
	manualset3
260845	3	424075	15	NULL	NULL	NULL	NULL	eradication	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacillary white diarrhoea of poultry and its eradication in the Union of South Africa .
	manualset3
260847	4	424075	15	NULL	NULL	NULL	NULL	Union of South Africa	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacillary white diarrhoea of poultry and its eradication in the Union of South Africa .
	manualset3
260850	1	424076	15	NULL	NULL	NULL	NULL	Bacille Calmette-Gurin ( BCG ) vaccines	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacille Calmette-Gurin ( BCG ) vaccines are widely used , even though estimates of efficacy have ranged from zero to 80 % .
	manualset3
260853	2	424076	15	NULL	NULL	NULL	NULL	estimates of efficacy	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacille Calmette-Gurin ( BCG ) vaccines are widely used , even though estimates of efficacy have ranged from zero to 80 % .
	manualset3
260855	3	424076	15	NULL	NULL	NULL	NULL	zero%	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacille Calmette-Gurin ( BCG ) vaccines are widely used , even though estimates of efficacy have ranged from zero to 80 % .
	manualset3
260856	4	424076	15	NULL	NULL	NULL	NULL	80 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacille Calmette-Gurin ( BCG ) vaccines are widely used , even though estimates of efficacy have ranged from zero to 80 % .
	manualset3
260882	1	424077	15	NULL	NULL	NULL	NULL	Experience	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experience with the management of premature labor ) .
	manualset3
260883	2	424077	15	NULL	NULL	NULL	NULL	management of premature labor	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experience with the management of premature labor ) .
	manualset3
260884	1	424078	15	NULL	NULL	NULL	NULL	Back-transforming	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Back-transforming the obtained expressions , a set of simple explicit expressions has been obtained that allow to directly obtain the intra-particle diffusion coefficient ( D ( part ) ) from peak parking or B-term constant measurements .
	manualset3
260885	2	424078	15	NULL	NULL	NULL	NULL	expressions	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Back-transforming the obtained expressions , a set of simple explicit expressions has been obtained that allow to directly obtain the intra-particle diffusion coefficient ( D ( part ) ) from peak parking or B-term constant measurements .
	manualset3
260886	3	424078	15	NULL	NULL	NULL	NULL	set	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Back-transforming the obtained expressions , a set of simple explicit expressions has been obtained that allow to directly obtain the intra-particle diffusion coefficient ( D ( part ) ) from peak parking or B-term constant measurements .
	manualset3
260887	4	424078	15	NULL	NULL	NULL	NULL	simple explicit expressions	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Back-transforming the obtained expressions , a set of simple explicit expressions has been obtained that allow to directly obtain the intra-particle diffusion coefficient ( D ( part ) ) from peak parking or B-term constant measurements .
	manualset3
260888	5	424078	15	NULL	NULL	NULL	NULL	intra-particle diffusion coefficient	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Back-transforming the obtained expressions , a set of simple explicit expressions has been obtained that allow to directly obtain the intra-particle diffusion coefficient ( D ( part ) ) from peak parking or B-term constant measurements .
	manualset3
260889	6	424078	15	NULL	NULL	NULL	NULL	D ( part )	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Back-transforming the obtained expressions , a set of simple explicit expressions has been obtained that allow to directly obtain the intra-particle diffusion coefficient ( D ( part ) ) from peak parking or B-term constant measurements .
	manualset3
260890	7	424078	15	NULL	NULL	NULL	NULL	peak parking	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Back-transforming the obtained expressions , a set of simple explicit expressions has been obtained that allow to directly obtain the intra-particle diffusion coefficient ( D ( part ) ) from peak parking or B-term constant measurements .
	manualset3
260891	8	424078	15	NULL	NULL	NULL	NULL	B-term constant measurements	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Back-transforming the obtained expressions , a set of simple explicit expressions has been obtained that allow to directly obtain the intra-particle diffusion coefficient ( D ( part ) ) from peak parking or B-term constant measurements .
	manualset3
260892	1	424079	15	NULL	NULL	NULL	NULL	future	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Back to the future in nursing ?
	manualset3
260893	2	424079	15	NULL	NULL	NULL	NULL	nursing	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Back to the future in nursing ?
	manualset3
260894	1	424080	15	NULL	NULL	NULL	NULL	Background	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Children with Prader-Willi syndrome ( PWS ) have decreased muscle mass , hypotonia , and impaired linear growth .
	manualset3
260895	2	424080	15	NULL	NULL	NULL	NULL	Children 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Children with Prader-Willi syndrome ( PWS ) have decreased muscle mass , hypotonia , and impaired linear growth .
	manualset3
260896	3	424080	15	NULL	NULL	NULL	NULL	Prader-Willi syndrome ( PWS )	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Children with Prader-Willi syndrome ( PWS ) have decreased muscle mass , hypotonia , and impaired linear growth .
	manualset3
260897	4	424080	15	NULL	NULL	NULL	NULL	decreased muscle mass	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Children with Prader-Willi syndrome ( PWS ) have decreased muscle mass , hypotonia , and impaired linear growth .
	manualset3
260898	5	424080	15	NULL	NULL	NULL	NULL	hypotonia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Children with Prader-Willi syndrome ( PWS ) have decreased muscle mass , hypotonia , and impaired linear growth .
	manualset3
260899	6	424080	15	NULL	NULL	NULL	NULL	impaired linear growth	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Children with Prader-Willi syndrome ( PWS ) have decreased muscle mass , hypotonia , and impaired linear growth .
	manualset3
260901	1	424081	15	NULL	NULL	NULL	NULL	Background	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Death from well-differentiated thyroid cancer ( WDTC ) is rare , and over the past century there has been a trend away from local recurrence as the primary cause of death .
	manualset3
260903	2	424081	15	NULL	NULL	NULL	NULL	Death	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Death from well-differentiated thyroid cancer ( WDTC ) is rare , and over the past century there has been a trend away from local recurrence as the primary cause of death .
	manualset3
260905	3	424081	15	NULL	NULL	NULL	NULL	well-differentiated thyroid cancer ( WDTC )	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Death from well-differentiated thyroid cancer ( WDTC ) is rare , and over the past century there has been a trend away from local recurrence as the primary cause of death .
	manualset3
260909	4	424081	15	NULL	NULL	NULL	NULL	over the past century	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Death from well-differentiated thyroid cancer ( WDTC ) is rare , and over the past century there has been a trend away from local recurrence as the primary cause of death .
	manualset3
260911	5	424081	15	NULL	NULL	NULL	NULL	trend	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Death from well-differentiated thyroid cancer ( WDTC ) is rare , and over the past century there has been a trend away from local recurrence as the primary cause of death .
	manualset3
260913	6	424081	15	NULL	NULL	NULL	NULL	local recurrence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Death from well-differentiated thyroid cancer ( WDTC ) is rare , and over the past century there has been a trend away from local recurrence as the primary cause of death .
	manualset3
260916	7	424081	15	NULL	NULL	NULL	NULL	primary cause of death	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Death from well-differentiated thyroid cancer ( WDTC ) is rare , and over the past century there has been a trend away from local recurrence as the primary cause of death .
	manualset3
260920	1	424082	15	NULL	NULL	NULL	NULL	Background	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Interferon-beta is used to reduce disease activity in multiple sclerosis , but its action is incompletely understood , individual treatment response varies among patients , and biological markers predicting clinical benefits have yet to be identified .
	manualset3
260921	2	424082	15	NULL	NULL	NULL	NULL	Interferon-beta	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Interferon-beta is used to reduce disease activity in multiple sclerosis , but its action is incompletely understood , individual treatment response varies among patients , and biological markers predicting clinical benefits have yet to be identified .
	manualset3
260922	3	424082	15	NULL	NULL	NULL	NULL	disease activity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Interferon-beta is used to reduce disease activity in multiple sclerosis , but its action is incompletely understood , individual treatment response varies among patients , and biological markers predicting clinical benefits have yet to be identified .
	manualset3
260923	4	424082	15	NULL	NULL	NULL	NULL	multiple sclerosis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Interferon-beta is used to reduce disease activity in multiple sclerosis , but its action is incompletely understood , individual treatment response varies among patients , and biological markers predicting clinical benefits have yet to be identified .
	manualset3
260924	5	424082	15	NULL	NULL	NULL	NULL	action	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Interferon-beta is used to reduce disease activity in multiple sclerosis , but its action is incompletely understood , individual treatment response varies among patients , and biological markers predicting clinical benefits have yet to be identified .
	manualset3
260925	6	424082	15	NULL	NULL	NULL	NULL	individual treatment response	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Interferon-beta is used to reduce disease activity in multiple sclerosis , but its action is incompletely understood , individual treatment response varies among patients , and biological markers predicting clinical benefits have yet to be identified .
	manualset3
260926	7	424082	15	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Interferon-beta is used to reduce disease activity in multiple sclerosis , but its action is incompletely understood , individual treatment response varies among patients , and biological markers predicting clinical benefits have yet to be identified .
	manualset3
260963	8	424082	15	NULL	NULL	NULL	NULL	biological markers 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Interferon-beta is used to reduce disease activity in multiple sclerosis , but its action is incompletely understood , individual treatment response varies among patients , and biological markers predicting clinical benefits have yet to be identified .
	manualset3
260965	9	424082	15	NULL	NULL	NULL	NULL	clinical benefits	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Interferon-beta is used to reduce disease activity in multiple sclerosis , but its action is incompletely understood , individual treatment response varies among patients , and biological markers predicting clinical benefits have yet to be identified .
	manualset3
260968	1	424083	15	NULL	NULL	NULL	NULL	Background	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : The `` biological susceptibility '' model posits that some individuals , by genetic predisposition , are highly sensitive to environmental stimuli .
	manualset3
260969	2	424083	15	NULL	NULL	NULL	NULL	` biological susceptibility '' model 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : The `` biological susceptibility '' model posits that some individuals , by genetic predisposition , are highly sensitive to environmental stimuli .
	manualset3
260970	3	424083	15	NULL	NULL	NULL	NULL	individuals 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : The `` biological susceptibility '' model posits that some individuals , by genetic predisposition , are highly sensitive to environmental stimuli .
	manualset3
260971	4	424083	15	NULL	NULL	NULL	NULL	genetic predisposition	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : The `` biological susceptibility '' model posits that some individuals , by genetic predisposition , are highly sensitive to environmental stimuli .
	manualset3
260972	5	424083	15	NULL	NULL	NULL	NULL	environmental stimuli 	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : The `` biological susceptibility '' model posits that some individuals , by genetic predisposition , are highly sensitive to environmental stimuli .
	manualset3
260976	1	424084	15	NULL	NULL	NULL	NULL	Background 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : The hemoglobincyanide method ( HiCN ) method for measuring hemoglobin is used extensively worldwide ; its advantages are the ready availability of a stable and internationally accepted reference standard calibrator .
	manualset3
260977	2	424084	15	NULL	NULL	NULL	NULL	hemoglobincyanide method ( HiCN ) method	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : The hemoglobincyanide method ( HiCN ) method for measuring hemoglobin is used extensively worldwide ; its advantages are the ready availability of a stable and internationally accepted reference standard calibrator .
	manualset3
260992	3	424084	15	NULL	NULL	NULL	NULL	measuring hemoglobin	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : The hemoglobincyanide method ( HiCN ) method for measuring hemoglobin is used extensively worldwide ; its advantages are the ready availability of a stable and internationally accepted reference standard calibrator .
	manualset3
260997	4	424084	15	NULL	NULL	NULL	NULL	advantages	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : The hemoglobincyanide method ( HiCN ) method for measuring hemoglobin is used extensively worldwide ; its advantages are the ready availability of a stable and internationally accepted reference standard calibrator .
	manualset3
261001	5	424084	15	NULL	NULL	NULL	NULL	availability	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : The hemoglobincyanide method ( HiCN ) method for measuring hemoglobin is used extensively worldwide ; its advantages are the ready availability of a stable and internationally accepted reference standard calibrator .
	manualset3
261004	6	424084	15	NULL	NULL	NULL	NULL	internationally accepted reference standard calibrator	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : The hemoglobincyanide method ( HiCN ) method for measuring hemoglobin is used extensively worldwide ; its advantages are the ready availability of a stable and internationally accepted reference standard calibrator .
	manualset3
261009	1	424085	15	NULL	NULL	NULL	NULL	Background 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background DYNC1H1 encodes the heavy chain protein of the cytoplasmic dynein 1 motor protein complex that plays a key role in retrograde axonal transport in neurons .
	manualset3
261011	2	424085	15	NULL	NULL	NULL	NULL	DYNC1H1	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background DYNC1H1 encodes the heavy chain protein of the cytoplasmic dynein 1 motor protein complex that plays a key role in retrograde axonal transport in neurons .
	manualset3
261013	3	424085	15	NULL	NULL	NULL	NULL	heavy chain protein	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background DYNC1H1 encodes the heavy chain protein of the cytoplasmic dynein 1 motor protein complex that plays a key role in retrograde axonal transport in neurons .
	manualset3
261014	4	424085	15	NULL	NULL	NULL	NULL	cytoplasmic dynein 1 motor protein complex	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background DYNC1H1 encodes the heavy chain protein of the cytoplasmic dynein 1 motor protein complex that plays a key role in retrograde axonal transport in neurons .
	manualset3
261016	5	424085	15	NULL	NULL	NULL	NULL	role	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background DYNC1H1 encodes the heavy chain protein of the cytoplasmic dynein 1 motor protein complex that plays a key role in retrograde axonal transport in neurons .
	manualset3
261018	6	424085	15	NULL	NULL	NULL	NULL	retrograde axonal transport	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background DYNC1H1 encodes the heavy chain protein of the cytoplasmic dynein 1 motor protein complex that plays a key role in retrograde axonal transport in neurons .
	manualset3
261020	7	424085	15	NULL	NULL	NULL	NULL	neurons	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background DYNC1H1 encodes the heavy chain protein of the cytoplasmic dynein 1 motor protein complex that plays a key role in retrograde axonal transport in neurons .
	manualset3
261021	1	424086	15	NULL	NULL	NULL	NULL	Experience	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experience with the use of guanethidine in arterial hypertension with special reference to its effects on the renal function and sodium excretion ) .
	manualset3
261023	2	424086	15	NULL	NULL	NULL	NULL	use	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experience with the use of guanethidine in arterial hypertension with special reference to its effects on the renal function and sodium excretion ) .
	manualset3
261025	3	424086	15	NULL	NULL	NULL	NULL	guanethidine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experience with the use of guanethidine in arterial hypertension with special reference to its effects on the renal function and sodium excretion ) .
	manualset3
261027	4	424086	15	NULL	NULL	NULL	NULL	arterial hypertension	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experience with the use of guanethidine in arterial hypertension with special reference to its effects on the renal function and sodium excretion ) .
	manualset3
261030	5	424086	15	NULL	NULL	NULL	NULL	reference	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experience with the use of guanethidine in arterial hypertension with special reference to its effects on the renal function and sodium excretion ) .
	manualset3
261033	6	424086	15	NULL	NULL	NULL	NULL	effects	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experience with the use of guanethidine in arterial hypertension with special reference to its effects on the renal function and sodium excretion ) .
	manualset3
261035	7	424086	15	NULL	NULL	NULL	NULL	renal function	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experience with the use of guanethidine in arterial hypertension with special reference to its effects on the renal function and sodium excretion ) .
	manualset3
261036	8	424086	15	NULL	NULL	NULL	NULL	sodium excretion	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experience with the use of guanethidine in arterial hypertension with special reference to its effects on the renal function and sodium excretion ) .
	manualset3
261037	1	424087	15	NULL	NULL	NULL	NULL	Background 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Demographic and clinical characteristics and angiographic findings of Turkish patients with coronary artery fistula have been investigated in this study and diagnostic tests and treatment methods used in these patients have also been evaluated in detail .
	manualset3
261041	2	424087	15	NULL	NULL	NULL	NULL	Demographic characteristics	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Demographic and clinical characteristics and angiographic findings of Turkish patients with coronary artery fistula have been investigated in this study and diagnostic tests and treatment methods used in these patients have also been evaluated in detail .
	manualset3
261043	3	424087	15	NULL	NULL	NULL	NULL	clinical characteristics	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Demographic and clinical characteristics and angiographic findings of Turkish patients with coronary artery fistula have been investigated in this study and diagnostic tests and treatment methods used in these patients have also been evaluated in detail .
	manualset3
261050	4	424087	15	NULL	NULL	NULL	NULL	angiographic findings 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Demographic and clinical characteristics and angiographic findings of Turkish patients with coronary artery fistula have been investigated in this study and diagnostic tests and treatment methods used in these patients have also been evaluated in detail .
	manualset3
261052	5	424087	15	NULL	NULL	NULL	NULL	Turkish patients 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Demographic and clinical characteristics and angiographic findings of Turkish patients with coronary artery fistula have been investigated in this study and diagnostic tests and treatment methods used in these patients have also been evaluated in detail .
	manualset3
261053	6	424087	15	NULL	NULL	NULL	NULL	coronary artery fistula	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Demographic and clinical characteristics and angiographic findings of Turkish patients with coronary artery fistula have been investigated in this study and diagnostic tests and treatment methods used in these patients have also been evaluated in detail .
	manualset3
261055	7	424087	15	NULL	NULL	NULL	NULL	study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Demographic and clinical characteristics and angiographic findings of Turkish patients with coronary artery fistula have been investigated in this study and diagnostic tests and treatment methods used in these patients have also been evaluated in detail .
	manualset3
261057	8	424087	15	NULL	NULL	NULL	NULL	diagnostic tests	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Demographic and clinical characteristics and angiographic findings of Turkish patients with coronary artery fistula have been investigated in this study and diagnostic tests and treatment methods used in these patients have also been evaluated in detail .
	manualset3
261059	9	424087	15	NULL	NULL	NULL	NULL	treatment methods	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Demographic and clinical characteristics and angiographic findings of Turkish patients with coronary artery fistula have been investigated in this study and diagnostic tests and treatment methods used in these patients have also been evaluated in detail .
	manualset3
261060	10	424087	15	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Demographic and clinical characteristics and angiographic findings of Turkish patients with coronary artery fistula have been investigated in this study and diagnostic tests and treatment methods used in these patients have also been evaluated in detail .
	manualset3
261062	11	424087	15	NULL	NULL	NULL	NULL	detail 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Demographic and clinical characteristics and angiographic findings of Turkish patients with coronary artery fistula have been investigated in this study and diagnostic tests and treatment methods used in these patients have also been evaluated in detail .
	manualset3
261068	1	424088	15	NULL	NULL	NULL	NULL	Background 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Effective and safe anticoagulative therapy needs close co-operation between doctor and patient , the latter being well-informed .
	manualset3
261069	2	424088	15	NULL	NULL	NULL	NULL	Effective anticoagulative therapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Effective and safe anticoagulative therapy needs close co-operation between doctor and patient , the latter being well-informed .
	manualset3
261071	3	424088	15	NULL	NULL	NULL	NULL	safe anticoagulative therapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Effective and safe anticoagulative therapy needs close co-operation between doctor and patient , the latter being well-informed .
	manualset3
261076	4	424088	15	NULL	NULL	NULL	NULL	co-operation	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Effective and safe anticoagulative therapy needs close co-operation between doctor and patient , the latter being well-informed .
	manualset3
261078	5	424088	15	NULL	NULL	NULL	NULL	doctor	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Effective and safe anticoagulative therapy needs close co-operation between doctor and patient , the latter being well-informed .
	manualset3
261080	6	424088	15	NULL	NULL	NULL	NULL	patient	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background : Effective and safe anticoagulative therapy needs close co-operation between doctor and patient , the latter being well-informed .
	manualset3
261087	1	424089	15	NULL	NULL	NULL	NULL	Background	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background/Aims : To assess the incidence of gastric cancer development in gastric benign ulcer patients and to evaluate the value of biopsy by taking specimens from both the base and edges of ulcers in contrast to the traditional biopsy which takes specimens from the edges of ulcers only .
	manualset3
261093	2	424089	15	NULL	NULL	NULL	NULL	Aims	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background/Aims : To assess the incidence of gastric cancer development in gastric benign ulcer patients and to evaluate the value of biopsy by taking specimens from both the base and edges of ulcers in contrast to the traditional biopsy which takes specimens from the edges of ulcers only .
	manualset3
261094	3	424089	15	NULL	NULL	NULL	NULL	incidence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background/Aims : To assess the incidence of gastric cancer development in gastric benign ulcer patients and to evaluate the value of biopsy by taking specimens from both the base and edges of ulcers in contrast to the traditional biopsy which takes specimens from the edges of ulcers only .
	manualset3
261101	5	424089	15	NULL	NULL	NULL	NULL	development	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background/Aims : To assess the incidence of gastric cancer development in gastric benign ulcer patients and to evaluate the value of biopsy by taking specimens from both the base and edges of ulcers in contrast to the traditional biopsy which takes specimens from the edges of ulcers only .
	manualset3
261103	6	424089	15	NULL	NULL	NULL	NULL	gastric benign ulcer patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background/Aims : To assess the incidence of gastric cancer development in gastric benign ulcer patients and to evaluate the value of biopsy by taking specimens from both the base and edges of ulcers in contrast to the traditional biopsy which takes specimens from the edges of ulcers only .
	manualset3
261105	7	424089	15	NULL	NULL	NULL	NULL	value of biopsy 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background/Aims : To assess the incidence of gastric cancer development in gastric benign ulcer patients and to evaluate the value of biopsy by taking specimens from both the base and edges of ulcers in contrast to the traditional biopsy which takes specimens from the edges of ulcers only .
	manualset3
261106	4	424089	15	NULL	NULL	NULL	NULL	gastric cancer	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background/Aims : To assess the incidence of gastric cancer development in gastric benign ulcer patients and to evaluate the value of biopsy by taking specimens from both the base and edges of ulcers in contrast to the traditional biopsy which takes specimens from the edges of ulcers only .
	manualset3
261107	8	424089	15	NULL	NULL	NULL	NULL	specimens	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background/Aims : To assess the incidence of gastric cancer development in gastric benign ulcer patients and to evaluate the value of biopsy by taking specimens from both the base and edges of ulcers in contrast to the traditional biopsy which takes specimens from the edges of ulcers only .
	manualset3
261108	9	424089	15	NULL	NULL	NULL	NULL	base of ulcers 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background/Aims : To assess the incidence of gastric cancer development in gastric benign ulcer patients and to evaluate the value of biopsy by taking specimens from both the base and edges of ulcers in contrast to the traditional biopsy which takes specimens from the edges of ulcers only .
	manualset3
261109	10	424089	15	NULL	NULL	NULL	NULL	edges of ulcers 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background/Aims : To assess the incidence of gastric cancer development in gastric benign ulcer patients and to evaluate the value of biopsy by taking specimens from both the base and edges of ulcers in contrast to the traditional biopsy which takes specimens from the edges of ulcers only .
	manualset3
261110	11	424089	15	NULL	NULL	NULL	NULL	traditional biopsy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background/Aims : To assess the incidence of gastric cancer development in gastric benign ulcer patients and to evaluate the value of biopsy by taking specimens from both the base and edges of ulcers in contrast to the traditional biopsy which takes specimens from the edges of ulcers only .
	manualset3
261111	12	424089	15	NULL	NULL	NULL	NULL	specimens	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background/Aims : To assess the incidence of gastric cancer development in gastric benign ulcer patients and to evaluate the value of biopsy by taking specimens from both the base and edges of ulcers in contrast to the traditional biopsy which takes specimens from the edges of ulcers only .
	manualset3
261112	13	424089	15	NULL	NULL	NULL	NULL	edges of ulcers	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Background/Aims : To assess the incidence of gastric cancer development in gastric benign ulcer patients and to evaluate the value of biopsy by taking specimens from both the base and edges of ulcers in contrast to the traditional biopsy which takes specimens from the edges of ulcers only .
	manualset3
261113	1	424090	15	NULL	NULL	NULL	NULL	Bacteria 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacteria grown on mineral salts-succinate with potassium nitrate gave responses to amino acids that were 2 to 3 times those of cells grown on ammonium sulfate and 10 to 20 times those of cells grown in mineral salts-succinate with Casamino Acids as the nitrogen source .
	manualset3
261114	2	424090	15	NULL	NULL	NULL	NULL	mineral salts-succinate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacteria grown on mineral salts-succinate with potassium nitrate gave responses to amino acids that were 2 to 3 times those of cells grown on ammonium sulfate and 10 to 20 times those of cells grown in mineral salts-succinate with Casamino Acids as the nitrogen source .
	manualset3
261115	3	424090	15	NULL	NULL	NULL	NULL	potassium nitrate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacteria grown on mineral salts-succinate with potassium nitrate gave responses to amino acids that were 2 to 3 times those of cells grown on ammonium sulfate and 10 to 20 times those of cells grown in mineral salts-succinate with Casamino Acids as the nitrogen source .
	manualset3
261116	4	424090	15	NULL	NULL	NULL	NULL	responses	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacteria grown on mineral salts-succinate with potassium nitrate gave responses to amino acids that were 2 to 3 times those of cells grown on ammonium sulfate and 10 to 20 times those of cells grown in mineral salts-succinate with Casamino Acids as the nitrogen source .
	manualset3
261117	5	424090	15	NULL	NULL	NULL	NULL	amino acids	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacteria grown on mineral salts-succinate with potassium nitrate gave responses to amino acids that were 2 to 3 times those of cells grown on ammonium sulfate and 10 to 20 times those of cells grown in mineral salts-succinate with Casamino Acids as the nitrogen source .
	manualset3
261120	6	424090	15	NULL	NULL	NULL	NULL	2 to 3 times 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacteria grown on mineral salts-succinate with potassium nitrate gave responses to amino acids that were 2 to 3 times those of cells grown on ammonium sulfate and 10 to 20 times those of cells grown in mineral salts-succinate with Casamino Acids as the nitrogen source .
	manualset3
261121	7	424090	15	NULL	NULL	NULL	NULL	cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacteria grown on mineral salts-succinate with potassium nitrate gave responses to amino acids that were 2 to 3 times those of cells grown on ammonium sulfate and 10 to 20 times those of cells grown in mineral salts-succinate with Casamino Acids as the nitrogen source .
	manualset3
261122	8	424090	15	NULL	NULL	NULL	NULL	ammonium sulfate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacteria grown on mineral salts-succinate with potassium nitrate gave responses to amino acids that were 2 to 3 times those of cells grown on ammonium sulfate and 10 to 20 times those of cells grown in mineral salts-succinate with Casamino Acids as the nitrogen source .
	manualset3
261123	9	424090	15	NULL	NULL	NULL	NULL	10 to 20 times 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacteria grown on mineral salts-succinate with potassium nitrate gave responses to amino acids that were 2 to 3 times those of cells grown on ammonium sulfate and 10 to 20 times those of cells grown in mineral salts-succinate with Casamino Acids as the nitrogen source .
	manualset3
261126	10	424090	15	NULL	NULL	NULL	NULL	cells 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacteria grown on mineral salts-succinate with potassium nitrate gave responses to amino acids that were 2 to 3 times those of cells grown on ammonium sulfate and 10 to 20 times those of cells grown in mineral salts-succinate with Casamino Acids as the nitrogen source .
	manualset3
261127	11	424090	15	NULL	NULL	NULL	NULL	mineral salts-succinate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacteria grown on mineral salts-succinate with potassium nitrate gave responses to amino acids that were 2 to 3 times those of cells grown on ammonium sulfate and 10 to 20 times those of cells grown in mineral salts-succinate with Casamino Acids as the nitrogen source .
	manualset3
261128	12	424090	15	NULL	NULL	NULL	NULL	Casamino Acids 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacteria grown on mineral salts-succinate with potassium nitrate gave responses to amino acids that were 2 to 3 times those of cells grown on ammonium sulfate and 10 to 20 times those of cells grown in mineral salts-succinate with Casamino Acids as the nitrogen source .
	manualset3
261129	13	424090	15	NULL	NULL	NULL	NULL	nitrogen source	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacteria grown on mineral salts-succinate with potassium nitrate gave responses to amino acids that were 2 to 3 times those of cells grown on ammonium sulfate and 10 to 20 times those of cells grown in mineral salts-succinate with Casamino Acids as the nitrogen source .
	manualset3
261130	1	424091	15	NULL	NULL	NULL	NULL	Bacteria 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacteria were also very potent inducers of DC maturation , although they enhanced the capacity of DCs to activate specific CD4 + T cells at concentrations that did not stimulate DC maturation .
	manualset3
261131	2	424091	15	NULL	NULL	NULL	NULL	inducers	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacteria were also very potent inducers of DC maturation , although they enhanced the capacity of DCs to activate specific CD4 + T cells at concentrations that did not stimulate DC maturation .
	manualset3
261132	3	424091	15	NULL	NULL	NULL	NULL	DC maturation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacteria were also very potent inducers of DC maturation , although they enhanced the capacity of DCs to activate specific CD4 + T cells at concentrations that did not stimulate DC maturation .
	manualset3
261133	4	424091	15	NULL	NULL	NULL	NULL	capacity of DCs	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacteria were also very potent inducers of DC maturation , although they enhanced the capacity of DCs to activate specific CD4 + T cells at concentrations that did not stimulate DC maturation .
	manualset3
261134	5	424091	15	NULL	NULL	NULL	NULL	CD4 + T cells 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacteria were also very potent inducers of DC maturation , although they enhanced the capacity of DCs to activate specific CD4 + T cells at concentrations that did not stimulate DC maturation .
	manualset3
261135	6	424091	15	NULL	NULL	NULL	NULL	concentrations	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacteria were also very potent inducers of DC maturation , although they enhanced the capacity of DCs to activate specific CD4 + T cells at concentrations that did not stimulate DC maturation .
	manualset3
261136	7	424091	15	NULL	NULL	NULL	NULL	DC maturation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacteria were also very potent inducers of DC maturation , although they enhanced the capacity of DCs to activate specific CD4 + T cells at concentrations that did not stimulate DC maturation .
	manualset3
261137	1	424092	15	NULL	NULL	NULL	NULL	Bacterial 16S ribosomal DNA ( rRNA ) gene PCR products	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacterial 16S ribosomal DNA ( rRNA ) gene PCR products were amplified from extracted nucleic acids , with analyses by terminal restriction fragment length polymorphism ( T-RFLP ) , length heterogeneity PCR ( LH-PCR ) , and sequencing of individual cloned PCR products to characterize these communities .
	manualset3
261138	2	424092	15	NULL	NULL	NULL	NULL	extracted nucleic acids	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacterial 16S ribosomal DNA ( rRNA ) gene PCR products were amplified from extracted nucleic acids , with analyses by terminal restriction fragment length polymorphism ( T-RFLP ) , length heterogeneity PCR ( LH-PCR ) , and sequencing of individual cloned PCR products to characterize these communities .
	manualset3
261154	3	424092	15	NULL	NULL	NULL	NULL	analyses	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacterial 16S ribosomal DNA ( rRNA ) gene PCR products were amplified from extracted nucleic acids , with analyses by terminal restriction fragment length polymorphism ( T-RFLP ) , length heterogeneity PCR ( LH-PCR ) , and sequencing of individual cloned PCR products to characterize these communities .
	manualset3
261155	4	424092	15	NULL	NULL	NULL	NULL	terminal restriction fragment length polymorphism ( T-RFLP ) 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacterial 16S ribosomal DNA ( rRNA ) gene PCR products were amplified from extracted nucleic acids , with analyses by terminal restriction fragment length polymorphism ( T-RFLP ) , length heterogeneity PCR ( LH-PCR ) , and sequencing of individual cloned PCR products to characterize these communities .
	manualset3
261156	5	424092	15	NULL	NULL	NULL	NULL	length heterogeneity PCR ( LH-PCR )	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacterial 16S ribosomal DNA ( rRNA ) gene PCR products were amplified from extracted nucleic acids , with analyses by terminal restriction fragment length polymorphism ( T-RFLP ) , length heterogeneity PCR ( LH-PCR ) , and sequencing of individual cloned PCR products to characterize these communities .
	manualset3
261157	6	424092	15	NULL	NULL	NULL	NULL	sequencing of individual cloned PCR products 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacterial 16S ribosomal DNA ( rRNA ) gene PCR products were amplified from extracted nucleic acids , with analyses by terminal restriction fragment length polymorphism ( T-RFLP ) , length heterogeneity PCR ( LH-PCR ) , and sequencing of individual cloned PCR products to characterize these communities .
	manualset3
261158	7	424092	15	NULL	NULL	NULL	NULL	communities 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacterial 16S ribosomal DNA ( rRNA ) gene PCR products were amplified from extracted nucleic acids , with analyses by terminal restriction fragment length polymorphism ( T-RFLP ) , length heterogeneity PCR ( LH-PCR ) , and sequencing of individual cloned PCR products to characterize these communities .
	manualset3
261290	1	424093	15	NULL	NULL	NULL	NULL	Bacterial biofilms	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacterial biofilms in chronic rhinosinusitis and their relationship with inflammation severity .
	manualset3
261291	2	424093	15	NULL	NULL	NULL	NULL	chronic rhinosinusitis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacterial biofilms in chronic rhinosinusitis and their relationship with inflammation severity .
	manualset3
261292	3	424093	15	NULL	NULL	NULL	NULL	relationship	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacterial biofilms in chronic rhinosinusitis and their relationship with inflammation severity .
	manualset3
261293	4	424093	15	NULL	NULL	NULL	NULL	inflammation severity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacterial biofilms in chronic rhinosinusitis and their relationship with inflammation severity .
	manualset3
261294	1	424094	15	NULL	NULL	NULL	NULL	Experiences	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experiences with butazolidin therapy of acute superficial thrombophlebitis after 2000 injections ) .
	manualset3
261295	2	424094	15	NULL	NULL	NULL	NULL	butazolidin therapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experiences with butazolidin therapy of acute superficial thrombophlebitis after 2000 injections ) .
	manualset3
261296	3	424094	15	NULL	NULL	NULL	NULL	acute superficial thrombophlebitis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experiences with butazolidin therapy of acute superficial thrombophlebitis after 2000 injections ) .
	manualset3
261297	4	424094	15	NULL	NULL	NULL	NULL	2000 injections 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experiences with butazolidin therapy of acute superficial thrombophlebitis after 2000 injections ) .
	manualset3
261298	1	424095	15	NULL	NULL	NULL	NULL	Bacterial isolates 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacterial isolates like P. fluorescens , Corynebacterium sp .
	manualset3
261299	2	424095	15	NULL	NULL	NULL	NULL	P. fluorescens	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacterial isolates like P. fluorescens , Corynebacterium sp .
	manualset3
261300	3	424095	15	NULL	NULL	NULL	NULL	Corynebacterium sp 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacterial isolates like P. fluorescens , Corynebacterium sp .
	manualset3
261301	1	424096	15	NULL	NULL	NULL	NULL	Bacteriophage SPP1 Chu	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacteriophage SPP1 Chu is an alkaline exonuclease in the SynExo family of viral two-component recombinases .
	manualset3
261302	2	424096	15	NULL	NULL	NULL	NULL	alkaline exonuclease	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacteriophage SPP1 Chu is an alkaline exonuclease in the SynExo family of viral two-component recombinases .
	manualset3
261303	3	424096	15	NULL	NULL	NULL	NULL	SynExo family 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacteriophage SPP1 Chu is an alkaline exonuclease in the SynExo family of viral two-component recombinases .
	manualset3
261304	4	424096	15	NULL	NULL	NULL	NULL	viral two-component recombinases	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bacteriophage SPP1 Chu is an alkaline exonuclease in the SynExo family of viral two-component recombinases .
	manualset3
261305	1	424097	15	NULL	NULL	NULL	NULL	Bactrocera dorsalis 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bactrocera dorsalis and Bactrocera zonata were studied under the effect of lead acetate for 48 hours exposure at larval stages .
	manualset3
261306	2	424097	15	NULL	NULL	NULL	NULL	Bactrocera zonata 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bactrocera dorsalis and Bactrocera zonata were studied under the effect of lead acetate for 48 hours exposure at larval stages .
	manualset3
261307	3	424097	15	NULL	NULL	NULL	NULL	effect	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bactrocera dorsalis and Bactrocera zonata were studied under the effect of lead acetate for 48 hours exposure at larval stages .
	manualset3
261308	4	424097	15	NULL	NULL	NULL	NULL	lead acetate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bactrocera dorsalis and Bactrocera zonata were studied under the effect of lead acetate for 48 hours exposure at larval stages .
	manualset3
261309	5	424097	15	NULL	NULL	NULL	NULL	48 hours exposure	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bactrocera dorsalis and Bactrocera zonata were studied under the effect of lead acetate for 48 hours exposure at larval stages .
	manualset3
261310	6	424097	15	NULL	NULL	NULL	NULL	larval stages	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bactrocera dorsalis and Bactrocera zonata were studied under the effect of lead acetate for 48 hours exposure at larval stages .
	manualset3
261311	1	424098	15	NULL	NULL	NULL	NULL	Baker	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baker induces apoptosis in HL-60 cells .
	manualset3
261312	2	424098	15	NULL	NULL	NULL	NULL	apoptosis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baker induces apoptosis in HL-60 cells .
	manualset3
261313	3	424098	15	NULL	NULL	NULL	NULL	HL-60 cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baker induces apoptosis in HL-60 cells .
	manualset3
261314	1	424099	15	NULL	NULL	NULL	NULL	rapid detoxification pathway	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Balancing this rapid detoxification pathway is endogenous formation from normal metabolic processes and exogenous formaldehyde input , resulting in approximately 0.1 mM systemic levels .
	manualset3
261315	2	424099	15	NULL	NULL	NULL	NULL	endogenous formation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Balancing this rapid detoxification pathway is endogenous formation from normal metabolic processes and exogenous formaldehyde input , resulting in approximately 0.1 mM systemic levels .
	manualset3
261316	3	424099	15	NULL	NULL	NULL	NULL	metabolic processes 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Balancing this rapid detoxification pathway is endogenous formation from normal metabolic processes and exogenous formaldehyde input , resulting in approximately 0.1 mM systemic levels .
	manualset3
261317	4	424099	15	NULL	NULL	NULL	NULL	exogenous formaldehyde input	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Balancing this rapid detoxification pathway is endogenous formation from normal metabolic processes and exogenous formaldehyde input , resulting in approximately 0.1 mM systemic levels .
	manualset3
261318	5	424099	15	NULL	NULL	NULL	NULL	0.1 mM	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Balancing this rapid detoxification pathway is endogenous formation from normal metabolic processes and exogenous formaldehyde input , resulting in approximately 0.1 mM systemic levels .
	manualset3
261319	6	424099	15	NULL	NULL	NULL	NULL	systemic levels	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Balancing this rapid detoxification pathway is endogenous formation from normal metabolic processes and exogenous formaldehyde input , resulting in approximately 0.1 mM systemic levels .
	manualset3
261320	1	424100	15	NULL	NULL	NULL	NULL	Balloon angioplasty 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Balloon angioplasty provides substantial anatomic and hemodynamic benefit in approximately 50 to 60 per cent of children with peripheral pulmonary artery stenosis .
	manualset3
261321	2	424100	15	NULL	NULL	NULL	NULL	anatomic benefit 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Balloon angioplasty provides substantial anatomic and hemodynamic benefit in approximately 50 to 60 per cent of children with peripheral pulmonary artery stenosis .
	manualset3
261322	3	424100	15	NULL	NULL	NULL	NULL	hemodynamic benefit	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Balloon angioplasty provides substantial anatomic and hemodynamic benefit in approximately 50 to 60 per cent of children with peripheral pulmonary artery stenosis .
	manualset3
261323	4	424100	15	NULL	NULL	NULL	NULL	50 to 60 per cent	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Balloon angioplasty provides substantial anatomic and hemodynamic benefit in approximately 50 to 60 per cent of children with peripheral pulmonary artery stenosis .
	manualset3
261324	5	424100	15	NULL	NULL	NULL	NULL	children	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Balloon angioplasty provides substantial anatomic and hemodynamic benefit in approximately 50 to 60 per cent of children with peripheral pulmonary artery stenosis .
	manualset3
261325	6	424100	15	NULL	NULL	NULL	NULL	peripheral pulmonary artery stenosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Balloon angioplasty provides substantial anatomic and hemodynamic benefit in approximately 50 to 60 per cent of children with peripheral pulmonary artery stenosis .
	manualset3
261326	1	424101	15	NULL	NULL	NULL	NULL	Balloon dilation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Balloon dilation facilitates stapling in esophagojejunostomy .
	manualset3
261352	2	424101	15	NULL	NULL	NULL	NULL	stapling	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Balloon dilation facilitates stapling in esophagojejunostomy .
	manualset3
261354	3	424101	15	NULL	NULL	NULL	NULL	esophagojejunostomy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Balloon dilation facilitates stapling in esophagojejunostomy .
	manualset3
261357	1	424102	15	NULL	NULL	NULL	NULL	Experiences	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experiences with the CM snap attachment ) .
	manualset3
261413	2	424102	15	NULL	NULL	NULL	NULL	CM snap attachment	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experiences with the CM snap attachment ) .
	manualset3
261361	1	424103	15	NULL	NULL	NULL	NULL	Band shift analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Band shift analysis at several elevated pressures found the equilibrium dissociation ( K ( d ) ) constant to be dependent on pressure , which allowed the volume change of dissociation ( deltaV ) to be calculated .
	manualset3
261362	2	424103	15	NULL	NULL	NULL	NULL	pressures 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Band shift analysis at several elevated pressures found the equilibrium dissociation ( K ( d ) ) constant to be dependent on pressure , which allowed the volume change of dissociation ( deltaV ) to be calculated .
	manualset3
261363	3	424103	15	NULL	NULL	NULL	NULL	equilibrium dissociation ( K ( d ) ) constant	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Band shift analysis at several elevated pressures found the equilibrium dissociation ( K ( d ) ) constant to be dependent on pressure , which allowed the volume change of dissociation ( deltaV ) to be calculated .
	manualset3
261364	4	424103	15	NULL	NULL	NULL	NULL	pressure	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Band shift analysis at several elevated pressures found the equilibrium dissociation ( K ( d ) ) constant to be dependent on pressure , which allowed the volume change of dissociation ( deltaV ) to be calculated .
	manualset3
261365	5	424103	15	NULL	NULL	NULL	NULL	volume change of dissociation ( deltaV )	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Band shift analysis at several elevated pressures found the equilibrium dissociation ( K ( d ) ) constant to be dependent on pressure , which allowed the volume change of dissociation ( deltaV ) to be calculated .
	manualset3
261366	1	424104	15	NULL	NULL	NULL	NULL	Barium hydroxide saline Giemsa staining	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Barium hydroxide saline Giemsa staining was used to examine heterochromatin polymorphism of chromosomes 1 , 9 and 16 in lymphocyte cultures .
	manualset3
261367	2	424104	15	NULL	NULL	NULL	NULL	heterochromatin polymorphism	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Barium hydroxide saline Giemsa staining was used to examine heterochromatin polymorphism of chromosomes 1 , 9 and 16 in lymphocyte cultures .
	manualset3
261368	3	424104	15	NULL	NULL	NULL	NULL	chromosomes 1	Chromosome												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Barium hydroxide saline Giemsa staining was used to examine heterochromatin polymorphism of chromosomes 1 , 9 and 16 in lymphocyte cultures .
	manualset3
261369	4	424104	15	NULL	NULL	NULL	NULL	chromosomes 9 	Chromosome												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Barium hydroxide saline Giemsa staining was used to examine heterochromatin polymorphism of chromosomes 1 , 9 and 16 in lymphocyte cultures .
	manualset3
261370	5	424104	15	NULL	NULL	NULL	NULL	chromosome 16	Chromosome												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Barium hydroxide saline Giemsa staining was used to examine heterochromatin polymorphism of chromosomes 1 , 9 and 16 in lymphocyte cultures .
	manualset3
261371	6	424104	15	NULL	NULL	NULL	NULL	lymphocyte cultures	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Barium hydroxide saline Giemsa staining was used to examine heterochromatin polymorphism of chromosomes 1 , 9 and 16 in lymphocyte cultures .
	manualset3
261372	1	424105	15	NULL	NULL	NULL	NULL	Barrett 's esophagus	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Barrett 's esophagus is considered to be a premalignant condition , and long-term surveillance seems mandatory with a careful search for dysplasia and carcinoma by means of multiple and repeated sets of biopsies .
	manualset3
261373	2	424105	15	NULL	NULL	NULL	NULL	premalignant condition	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Barrett 's esophagus is considered to be a premalignant condition , and long-term surveillance seems mandatory with a careful search for dysplasia and carcinoma by means of multiple and repeated sets of biopsies .
	manualset3
261374	3	424105	15	NULL	NULL	NULL	NULL	long-term surveillance	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Barrett 's esophagus is considered to be a premalignant condition , and long-term surveillance seems mandatory with a careful search for dysplasia and carcinoma by means of multiple and repeated sets of biopsies .
	manualset3
261375	4	424105	15	NULL	NULL	NULL	NULL	search	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Barrett 's esophagus is considered to be a premalignant condition , and long-term surveillance seems mandatory with a careful search for dysplasia and carcinoma by means of multiple and repeated sets of biopsies .
	manualset3
261376	5	424105	15	NULL	NULL	NULL	NULL	dysplasia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Barrett 's esophagus is considered to be a premalignant condition , and long-term surveillance seems mandatory with a careful search for dysplasia and carcinoma by means of multiple and repeated sets of biopsies .
	manualset3
261377	6	424105	15	NULL	NULL	NULL	NULL	carcinoma	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Barrett 's esophagus is considered to be a premalignant condition , and long-term surveillance seems mandatory with a careful search for dysplasia and carcinoma by means of multiple and repeated sets of biopsies .
	manualset3
261378	7	424105	15	NULL	NULL	NULL	NULL	multiple sets of biopsies	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Barrett 's esophagus is considered to be a premalignant condition , and long-term surveillance seems mandatory with a careful search for dysplasia and carcinoma by means of multiple and repeated sets of biopsies .
	manualset3
261379	8	424105	15	NULL	NULL	NULL	NULL	repeated sets of biopsies	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Barrett 's esophagus is considered to be a premalignant condition , and long-term surveillance seems mandatory with a careful search for dysplasia and carcinoma by means of multiple and repeated sets of biopsies .
	manualset3
261380	1	424106	15	NULL	NULL	NULL	NULL	Basal IGF-I level	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal IGF-I level was below 10 ng/ml in all patients except one .
	manualset3
261381	2	424106	15	NULL	NULL	NULL	NULL	10 ng/ml	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal IGF-I level was below 10 ng/ml in all patients except one .
	manualset3
261382	3	424106	15	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal IGF-I level was below 10 ng/ml in all patients except one .
	manualset3
261383	4	424106	15	NULL	NULL	NULL	NULL	one	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal IGF-I level was below 10 ng/ml in all patients except one .
	manualset3
261384	1	424107	15	NULL	NULL	NULL	NULL	Basal serum TSH concentrations	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal and TRH-induced serum TSH concentrations in young males are significantly ( P less than .05 ) higher than in old males , while there is no significant difference in basal TSH between young and old female rats , but young females had greater TSH response to TRH than the old females .
	manualset3
261385	2	424107	15	NULL	NULL	NULL	NULL	TRH-induced serum TSH concentrations	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal and TRH-induced serum TSH concentrations in young males are significantly ( P less than .05 ) higher than in old males , while there is no significant difference in basal TSH between young and old female rats , but young females had greater TSH response to TRH than the old females .
	manualset3
261386	3	424107	15	NULL	NULL	NULL	NULL	young males	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal and TRH-induced serum TSH concentrations in young males are significantly ( P less than .05 ) higher than in old males , while there is no significant difference in basal TSH between young and old female rats , but young females had greater TSH response to TRH than the old females .
	manualset3
261387	4	424107	15	NULL	NULL	NULL	NULL	P less than .05	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal and TRH-induced serum TSH concentrations in young males are significantly ( P less than .05 ) higher than in old males , while there is no significant difference in basal TSH between young and old female rats , but young females had greater TSH response to TRH than the old females .
	manualset3
261388	5	424107	15	NULL	NULL	NULL	NULL	old males	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal and TRH-induced serum TSH concentrations in young males are significantly ( P less than .05 ) higher than in old males , while there is no significant difference in basal TSH between young and old female rats , but young females had greater TSH response to TRH than the old females .
	manualset3
261389	6	424107	15	NULL	NULL	NULL	NULL	significant difference	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal and TRH-induced serum TSH concentrations in young males are significantly ( P less than .05 ) higher than in old males , while there is no significant difference in basal TSH between young and old female rats , but young females had greater TSH response to TRH than the old females .
	manualset3
261390	7	424107	15	NULL	NULL	NULL	NULL	TSH	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal and TRH-induced serum TSH concentrations in young males are significantly ( P less than .05 ) higher than in old males , while there is no significant difference in basal TSH between young and old female rats , but young females had greater TSH response to TRH than the old females .
	manualset3
261391	8	424107	15	NULL	NULL	NULL	NULL	young female rats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal and TRH-induced serum TSH concentrations in young males are significantly ( P less than .05 ) higher than in old males , while there is no significant difference in basal TSH between young and old female rats , but young females had greater TSH response to TRH than the old females .
	manualset3
261392	9	424107	15	NULL	NULL	NULL	NULL	old female rats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal and TRH-induced serum TSH concentrations in young males are significantly ( P less than .05 ) higher than in old males , while there is no significant difference in basal TSH between young and old female rats , but young females had greater TSH response to TRH than the old females .
	manualset3
261393	10	424107	15	NULL	NULL	NULL	NULL	young females	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal and TRH-induced serum TSH concentrations in young males are significantly ( P less than .05 ) higher than in old males , while there is no significant difference in basal TSH between young and old female rats , but young females had greater TSH response to TRH than the old females .
	manualset3
261394	11	424107	15	NULL	NULL	NULL	NULL	TSH response	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal and TRH-induced serum TSH concentrations in young males are significantly ( P less than .05 ) higher than in old males , while there is no significant difference in basal TSH between young and old female rats , but young females had greater TSH response to TRH than the old females .
	manualset3
261395	12	424107	15	NULL	NULL	NULL	NULL	TRH	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal and TRH-induced serum TSH concentrations in young males are significantly ( P less than .05 ) higher than in old males , while there is no significant difference in basal TSH between young and old female rats , but young females had greater TSH response to TRH than the old females .
	manualset3
261396	13	424107	15	NULL	NULL	NULL	NULL	old females	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal and TRH-induced serum TSH concentrations in young males are significantly ( P less than .05 ) higher than in old males , while there is no significant difference in basal TSH between young and old female rats , but young females had greater TSH response to TRH than the old females .
	manualset3
261397	1	424108	15	NULL	NULL	NULL	NULL	Basal laser Doppler flux ( BLDF )	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal laser Doppler flux ( BLDF ) , amplitude of vasomotion waves ( AV ) , post-occlusive reactive hyperthermia peakflow ( F Max ) , difference between BLDF and F Max ( delta F Max ) , time to reach 50 percent of the initial value ( t1/2 r ) and total recovery ( tr ) , t Max ( peak of over-shoot ) and t/2 over shoot were measured .
	manualset3
261398	2	424108	15	NULL	NULL	NULL	NULL	amplitude of vasomotion waves ( AV )	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal laser Doppler flux ( BLDF ) , amplitude of vasomotion waves ( AV ) , post-occlusive reactive hyperthermia peakflow ( F Max ) , difference between BLDF and F Max ( delta F Max ) , time to reach 50 percent of the initial value ( t1/2 r ) and total recovery ( tr ) , t Max ( peak of over-shoot ) and t/2 over shoot were measured .
	manualset3
261399	3	424108	15	NULL	NULL	NULL	NULL	post-occlusive reactive hyperthermia peakflow ( F Max )	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal laser Doppler flux ( BLDF ) , amplitude of vasomotion waves ( AV ) , post-occlusive reactive hyperthermia peakflow ( F Max ) , difference between BLDF and F Max ( delta F Max ) , time to reach 50 percent of the initial value ( t1/2 r ) and total recovery ( tr ) , t Max ( peak of over-shoot ) and t/2 over shoot were measured .
	manualset3
261400	4	424108	15	NULL	NULL	NULL	NULL	difference	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal laser Doppler flux ( BLDF ) , amplitude of vasomotion waves ( AV ) , post-occlusive reactive hyperthermia peakflow ( F Max ) , difference between BLDF and F Max ( delta F Max ) , time to reach 50 percent of the initial value ( t1/2 r ) and total recovery ( tr ) , t Max ( peak of over-shoot ) and t/2 over shoot were measured .
	manualset3
261401	5	424108	15	NULL	NULL	NULL	NULL	BLDF	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal laser Doppler flux ( BLDF ) , amplitude of vasomotion waves ( AV ) , post-occlusive reactive hyperthermia peakflow ( F Max ) , difference between BLDF and F Max ( delta F Max ) , time to reach 50 percent of the initial value ( t1/2 r ) and total recovery ( tr ) , t Max ( peak of over-shoot ) and t/2 over shoot were measured .
	manualset3
261402	6	424108	15	NULL	NULL	NULL	NULL	F Max ( delta F Max )	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal laser Doppler flux ( BLDF ) , amplitude of vasomotion waves ( AV ) , post-occlusive reactive hyperthermia peakflow ( F Max ) , difference between BLDF and F Max ( delta F Max ) , time to reach 50 percent of the initial value ( t1/2 r ) and total recovery ( tr ) , t Max ( peak of over-shoot ) and t/2 over shoot were measured .
	manualset3
261403	7	424108	15	NULL	NULL	NULL	NULL	time	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal laser Doppler flux ( BLDF ) , amplitude of vasomotion waves ( AV ) , post-occlusive reactive hyperthermia peakflow ( F Max ) , difference between BLDF and F Max ( delta F Max ) , time to reach 50 percent of the initial value ( t1/2 r ) and total recovery ( tr ) , t Max ( peak of over-shoot ) and t/2 over shoot were measured .
	manualset3
261404	8	424108	15	NULL	NULL	NULL	NULL	50 percent	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal laser Doppler flux ( BLDF ) , amplitude of vasomotion waves ( AV ) , post-occlusive reactive hyperthermia peakflow ( F Max ) , difference between BLDF and F Max ( delta F Max ) , time to reach 50 percent of the initial value ( t1/2 r ) and total recovery ( tr ) , t Max ( peak of over-shoot ) and t/2 over shoot were measured .
	manualset3
261405	9	424108	15	NULL	NULL	NULL	NULL	initial value ( t1/2 r ) 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal laser Doppler flux ( BLDF ) , amplitude of vasomotion waves ( AV ) , post-occlusive reactive hyperthermia peakflow ( F Max ) , difference between BLDF and F Max ( delta F Max ) , time to reach 50 percent of the initial value ( t1/2 r ) and total recovery ( tr ) , t Max ( peak of over-shoot ) and t/2 over shoot were measured .
	manualset3
261406	10	424108	15	NULL	NULL	NULL	NULL	total recovery ( tr )	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal laser Doppler flux ( BLDF ) , amplitude of vasomotion waves ( AV ) , post-occlusive reactive hyperthermia peakflow ( F Max ) , difference between BLDF and F Max ( delta F Max ) , time to reach 50 percent of the initial value ( t1/2 r ) and total recovery ( tr ) , t Max ( peak of over-shoot ) and t/2 over shoot were measured .
	manualset3
261407	11	424108	15	NULL	NULL	NULL	NULL	t Max ( peak of over-shoot )	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal laser Doppler flux ( BLDF ) , amplitude of vasomotion waves ( AV ) , post-occlusive reactive hyperthermia peakflow ( F Max ) , difference between BLDF and F Max ( delta F Max ) , time to reach 50 percent of the initial value ( t1/2 r ) and total recovery ( tr ) , t Max ( peak of over-shoot ) and t/2 over shoot were measured .
	manualset3
261408	12	424108	15	NULL	NULL	NULL	NULL	t/2	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal laser Doppler flux ( BLDF ) , amplitude of vasomotion waves ( AV ) , post-occlusive reactive hyperthermia peakflow ( F Max ) , difference between BLDF and F Max ( delta F Max ) , time to reach 50 percent of the initial value ( t1/2 r ) and total recovery ( tr ) , t Max ( peak of over-shoot ) and t/2 over shoot were measured .
	manualset3
261409	13	424108	15	NULL	NULL	NULL	NULL	shoot	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal laser Doppler flux ( BLDF ) , amplitude of vasomotion waves ( AV ) , post-occlusive reactive hyperthermia peakflow ( F Max ) , difference between BLDF and F Max ( delta F Max ) , time to reach 50 percent of the initial value ( t1/2 r ) and total recovery ( tr ) , t Max ( peak of over-shoot ) and t/2 over shoot were measured .
	manualset3
261410	1	424109	15	NULL	NULL	NULL	NULL	Basal parameters	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal parameters for binding and cross-linking of 125I-rat prolactin ( rPRL ) to lactogenic ( PRL ) binding species present in crude membrane fraction ( CMF ) or detergent-solubilized preparations of rat liver have been investigated .
	manualset3
261411	2	424109	15	NULL	NULL	NULL	NULL	binding 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal parameters for binding and cross-linking of 125I-rat prolactin ( rPRL ) to lactogenic ( PRL ) binding species present in crude membrane fraction ( CMF ) or detergent-solubilized preparations of rat liver have been investigated .
	manualset3
261412	4	424109	15	NULL	NULL	NULL	NULL	125I-rat prolactin ( rPRL )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal parameters for binding and cross-linking of 125I-rat prolactin ( rPRL ) to lactogenic ( PRL ) binding species present in crude membrane fraction ( CMF ) or detergent-solubilized preparations of rat liver have been investigated .
	manualset3
261414	5	424109	15	NULL	NULL	NULL	NULL	lactogenic ( PRL ) binding species	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal parameters for binding and cross-linking of 125I-rat prolactin ( rPRL ) to lactogenic ( PRL ) binding species present in crude membrane fraction ( CMF ) or detergent-solubilized preparations of rat liver have been investigated .
	manualset3
261415	6	424109	15	NULL	NULL	NULL	NULL	crude membrane fraction ( CMF )	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal parameters for binding and cross-linking of 125I-rat prolactin ( rPRL ) to lactogenic ( PRL ) binding species present in crude membrane fraction ( CMF ) or detergent-solubilized preparations of rat liver have been investigated .
	manualset3
261416	7	424109	15	NULL	NULL	NULL	NULL	detergent-solubilized preparations of rat liver	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal parameters for binding and cross-linking of 125I-rat prolactin ( rPRL ) to lactogenic ( PRL ) binding species present in crude membrane fraction ( CMF ) or detergent-solubilized preparations of rat liver have been investigated .
	manualset3
261548	3	424109	15	NULL	NULL	NULL	NULL	cross-linking 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal parameters for binding and cross-linking of 125I-rat prolactin ( rPRL ) to lactogenic ( PRL ) binding species present in crude membrane fraction ( CMF ) or detergent-solubilized preparations of rat liver have been investigated .
	manualset3
261417	1	424110	15	NULL	NULL	NULL	NULL	Experiences	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experiences with the Filatov-therapy in urology ) .
	manualset3
261418	2	424110	15	NULL	NULL	NULL	NULL	Filatov-therapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experiences with the Filatov-therapy in urology ) .
	manualset3
261419	3	424110	15	NULL	NULL	NULL	NULL	urology	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experiences with the Filatov-therapy in urology ) .
	manualset3
261420	1	424111	15	NULL	NULL	NULL	NULL	Basal release	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal release in the hippocampus was not significantly different from the sham controls .
	manualset3
261421	2	424111	15	NULL	NULL	NULL	NULL	hippocampus	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal release in the hippocampus was not significantly different from the sham controls .
	manualset3
261422	3	424111	15	NULL	NULL	NULL	NULL	sham controls	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basal release in the hippocampus was not significantly different from the sham controls .
	manualset3
261423	1	424112	15	NULL	NULL	NULL	NULL	Base cations	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Base cations either decreased ( mean percentage decrease for calcium was 5.4 % year ( -1 ) and for magnesium 4.4 % year ( -1 ) ) or did not show any significant change ( sodium , potassium ) .
	manualset3
261424	2	424112	15	NULL	NULL	NULL	NULL	mean percentage decrease	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Base cations either decreased ( mean percentage decrease for calcium was 5.4 % year ( -1 ) and for magnesium 4.4 % year ( -1 ) ) or did not show any significant change ( sodium , potassium ) .
	manualset3
261425	3	424112	15	NULL	NULL	NULL	NULL	calcium	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Base cations either decreased ( mean percentage decrease for calcium was 5.4 % year ( -1 ) and for magnesium 4.4 % year ( -1 ) ) or did not show any significant change ( sodium , potassium ) .
	manualset3
261426	4	424112	15	NULL	NULL	NULL	NULL	5.4 % year ( -1 )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Base cations either decreased ( mean percentage decrease for calcium was 5.4 % year ( -1 ) and for magnesium 4.4 % year ( -1 ) ) or did not show any significant change ( sodium , potassium ) .
	manualset3
261427	5	424112	15	NULL	NULL	NULL	NULL	magnesium	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Base cations either decreased ( mean percentage decrease for calcium was 5.4 % year ( -1 ) and for magnesium 4.4 % year ( -1 ) ) or did not show any significant change ( sodium , potassium ) .
	manualset3
261428	6	424112	15	NULL	NULL	NULL	NULL	4.4 % year ( -1 )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Base cations either decreased ( mean percentage decrease for calcium was 5.4 % year ( -1 ) and for magnesium 4.4 % year ( -1 ) ) or did not show any significant change ( sodium , potassium ) .
	manualset3
261429	7	424112	15	NULL	NULL	NULL	NULL	significant change	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Base cations either decreased ( mean percentage decrease for calcium was 5.4 % year ( -1 ) and for magnesium 4.4 % year ( -1 ) ) or did not show any significant change ( sodium , potassium ) .
	manualset3
261430	8	424112	15	NULL	NULL	NULL	NULL	sodium	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Base cations either decreased ( mean percentage decrease for calcium was 5.4 % year ( -1 ) and for magnesium 4.4 % year ( -1 ) ) or did not show any significant change ( sodium , potassium ) .
	manualset3
261431	9	424112	15	NULL	NULL	NULL	NULL	potassium	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Base cations either decreased ( mean percentage decrease for calcium was 5.4 % year ( -1 ) and for magnesium 4.4 % year ( -1 ) ) or did not show any significant change ( sodium , potassium ) .
	manualset3
261432	1	424113	15	NULL	NULL	NULL	NULL	Base excision repair pathways	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Base excision and nucleotide excision repair pathways in mycobacteria .
	manualset3
261433	2	424113	15	NULL	NULL	NULL	NULL	nucleotide excision repair pathways	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Base excision and nucleotide excision repair pathways in mycobacteria .
	manualset3
261434	3	424113	15	NULL	NULL	NULL	NULL	mycobacteria	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Base excision and nucleotide excision repair pathways in mycobacteria .
	manualset3
261435	1	424114	15	NULL	NULL	NULL	NULL	LOECs	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Base on LOECs , our results indicated that histopathological endpoints are high sensitivity to copper and lithium compared to endpoints for embryonic developmental toxicity .
	manualset3
261436	2	424114	15	NULL	NULL	NULL	NULL	results	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Base on LOECs , our results indicated that histopathological endpoints are high sensitivity to copper and lithium compared to endpoints for embryonic developmental toxicity .
	manualset3
261437	3	424114	15	NULL	NULL	NULL	NULL	histopathological endpoints	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Base on LOECs , our results indicated that histopathological endpoints are high sensitivity to copper and lithium compared to endpoints for embryonic developmental toxicity .
	manualset3
261438	4	424114	15	NULL	NULL	NULL	NULL	sensitivity	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Base on LOECs , our results indicated that histopathological endpoints are high sensitivity to copper and lithium compared to endpoints for embryonic developmental toxicity .
	manualset3
261439	5	424114	15	NULL	NULL	NULL	NULL	copper	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Base on LOECs , our results indicated that histopathological endpoints are high sensitivity to copper and lithium compared to endpoints for embryonic developmental toxicity .
	manualset3
261440	6	424114	15	NULL	NULL	NULL	NULL	lithium	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Base on LOECs , our results indicated that histopathological endpoints are high sensitivity to copper and lithium compared to endpoints for embryonic developmental toxicity .
	manualset3
261441	7	424114	15	NULL	NULL	NULL	NULL	endpoints	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Base on LOECs , our results indicated that histopathological endpoints are high sensitivity to copper and lithium compared to endpoints for embryonic developmental toxicity .
	manualset3
261442	8	424114	15	NULL	NULL	NULL	NULL	embryonic developmental toxicity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Base on LOECs , our results indicated that histopathological endpoints are high sensitivity to copper and lithium compared to endpoints for embryonic developmental toxicity .
	manualset3
261443	1	424115	15	NULL	NULL	NULL	NULL	480 observations	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on 480 observations , the milk yields per lactation for the Holstein , Jersey and Brown Swiss sired groups were 2 , 821 + / - 163 , 2 , 320 + / - 61 and 2 , 418 + / - 119 kg , respectively .
	manualset3
261444	2	424115	15	NULL	NULL	NULL	NULL	milk yields per lactation	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on 480 observations , the milk yields per lactation for the Holstein , Jersey and Brown Swiss sired groups were 2 , 821 + / - 163 , 2 , 320 + / - 61 and 2 , 418 + / - 119 kg , respectively .
	manualset3
261445	3	424115	15	NULL	NULL	NULL	NULL	Holstein sired groups	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on 480 observations , the milk yields per lactation for the Holstein , Jersey and Brown Swiss sired groups were 2 , 821 + / - 163 , 2 , 320 + / - 61 and 2 , 418 + / - 119 kg , respectively .
	manualset3
261446	4	424115	15	NULL	NULL	NULL	NULL	Jersey sired groups	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on 480 observations , the milk yields per lactation for the Holstein , Jersey and Brown Swiss sired groups were 2 , 821 + / - 163 , 2 , 320 + / - 61 and 2 , 418 + / - 119 kg , respectively .
	manualset3
261447	5	424115	15	NULL	NULL	NULL	NULL	Brown Swiss sired groups	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on 480 observations , the milk yields per lactation for the Holstein , Jersey and Brown Swiss sired groups were 2 , 821 + / - 163 , 2 , 320 + / - 61 and 2 , 418 + / - 119 kg , respectively .
	manualset3
261448	6	424115	15	NULL	NULL	NULL	NULL	2 , 821 + / - 163 kg	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on 480 observations , the milk yields per lactation for the Holstein , Jersey and Brown Swiss sired groups were 2 , 821 + / - 163 , 2 , 320 + / - 61 and 2 , 418 + / - 119 kg , respectively .
	manualset3
261450	7	424115	15	NULL	NULL	NULL	NULL	2 , 320 + / - 61 kg	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on 480 observations , the milk yields per lactation for the Holstein , Jersey and Brown Swiss sired groups were 2 , 821 + / - 163 , 2 , 320 + / - 61 and 2 , 418 + / - 119 kg , respectively .
	manualset3
261451	8	424115	15	NULL	NULL	NULL	NULL	2 , 418 + / - 119 kg	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on 480 observations , the milk yields per lactation for the Holstein , Jersey and Brown Swiss sired groups were 2 , 821 + / - 163 , 2 , 320 + / - 61 and 2 , 418 + / - 119 kg , respectively .
	manualset3
261452	1	424116	15	NULL	NULL	NULL	NULL	DNA sequencing studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on DNA sequencing studies , this last codes for a hydrophobic protein of 415 amino acids .
	manualset3
261453	2	424116	15	NULL	NULL	NULL	NULL	hydrophobic protein	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on DNA sequencing studies , this last codes for a hydrophobic protein of 415 amino acids .
	manualset3
261454	3	424116	15	NULL	NULL	NULL	NULL	415	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on DNA sequencing studies , this last codes for a hydrophobic protein of 415 amino acids .
	manualset3
261455	4	424116	15	NULL	NULL	NULL	NULL	amino acids	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on DNA sequencing studies , this last codes for a hydrophobic protein of 415 amino acids .
	manualset3
261456	1	424117	15	NULL	NULL	NULL	NULL	semistructured psychiatric exam 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on a semistructured psychiatric exam and DSM-IV diagnostic criteria , a consecutive series of 23 patients who met criteria for major depression ( N = 16 ) or minor depression ( N = 7 ) were selected and randomly assigned to either active treatment ( nortriptyline ) or placebo .
	manualset3
261457	2	424117	15	NULL	NULL	NULL	NULL	DSM-IV diagnostic criteria	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on a semistructured psychiatric exam and DSM-IV diagnostic criteria , a consecutive series of 23 patients who met criteria for major depression ( N = 16 ) or minor depression ( N = 7 ) were selected and randomly assigned to either active treatment ( nortriptyline ) or placebo .
	manualset3
261458	3	424117	15	NULL	NULL	NULL	NULL	consecutive series 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on a semistructured psychiatric exam and DSM-IV diagnostic criteria , a consecutive series of 23 patients who met criteria for major depression ( N = 16 ) or minor depression ( N = 7 ) were selected and randomly assigned to either active treatment ( nortriptyline ) or placebo .
	manualset3
261459	4	424117	15	NULL	NULL	NULL	NULL	23 patients 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on a semistructured psychiatric exam and DSM-IV diagnostic criteria , a consecutive series of 23 patients who met criteria for major depression ( N = 16 ) or minor depression ( N = 7 ) were selected and randomly assigned to either active treatment ( nortriptyline ) or placebo .
	manualset3
261460	5	424117	15	NULL	NULL	NULL	NULL	criteria	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on a semistructured psychiatric exam and DSM-IV diagnostic criteria , a consecutive series of 23 patients who met criteria for major depression ( N = 16 ) or minor depression ( N = 7 ) were selected and randomly assigned to either active treatment ( nortriptyline ) or placebo .
	manualset3
261461	6	424117	15	NULL	NULL	NULL	NULL	major depression	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on a semistructured psychiatric exam and DSM-IV diagnostic criteria , a consecutive series of 23 patients who met criteria for major depression ( N = 16 ) or minor depression ( N = 7 ) were selected and randomly assigned to either active treatment ( nortriptyline ) or placebo .
	manualset3
261462	7	424117	15	NULL	NULL	NULL	NULL	N = 16	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on a semistructured psychiatric exam and DSM-IV diagnostic criteria , a consecutive series of 23 patients who met criteria for major depression ( N = 16 ) or minor depression ( N = 7 ) were selected and randomly assigned to either active treatment ( nortriptyline ) or placebo .
	manualset3
261463	8	424117	15	NULL	NULL	NULL	NULL	minor depression	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on a semistructured psychiatric exam and DSM-IV diagnostic criteria , a consecutive series of 23 patients who met criteria for major depression ( N = 16 ) or minor depression ( N = 7 ) were selected and randomly assigned to either active treatment ( nortriptyline ) or placebo .
	manualset3
261464	9	424117	15	NULL	NULL	NULL	NULL	N = 7 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on a semistructured psychiatric exam and DSM-IV diagnostic criteria , a consecutive series of 23 patients who met criteria for major depression ( N = 16 ) or minor depression ( N = 7 ) were selected and randomly assigned to either active treatment ( nortriptyline ) or placebo .
	manualset3
261465	10	424117	15	NULL	NULL	NULL	NULL	active treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on a semistructured psychiatric exam and DSM-IV diagnostic criteria , a consecutive series of 23 patients who met criteria for major depression ( N = 16 ) or minor depression ( N = 7 ) were selected and randomly assigned to either active treatment ( nortriptyline ) or placebo .
	manualset3
261466	11	424117	15	NULL	NULL	NULL	NULL	nortriptyline	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on a semistructured psychiatric exam and DSM-IV diagnostic criteria , a consecutive series of 23 patients who met criteria for major depression ( N = 16 ) or minor depression ( N = 7 ) were selected and randomly assigned to either active treatment ( nortriptyline ) or placebo .
	manualset3
261467	12	424117	15	NULL	NULL	NULL	NULL	placebo	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on a semistructured psychiatric exam and DSM-IV diagnostic criteria , a consecutive series of 23 patients who met criteria for major depression ( N = 16 ) or minor depression ( N = 7 ) were selected and randomly assigned to either active treatment ( nortriptyline ) or placebo .
	manualset3
261468	1	424118	15	NULL	NULL	NULL	NULL	variety	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on a variety of qualitative and quantitative considerations ( cf. Tate , C. A. , Bick , R. J. , Chu , A. , Van Winkle , W. B. , and Entman , M. L. ( 1985 ) J. Biol .
	manualset3
261469	2	424118	15	NULL	NULL	NULL	NULL	qualitative considerations 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on a variety of qualitative and quantitative considerations ( cf. Tate , C. A. , Bick , R. J. , Chu , A. , Van Winkle , W. B. , and Entman , M. L. ( 1985 ) J. Biol .
	manualset3
261470	3	424118	15	NULL	NULL	NULL	NULL	quantitative considerations 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on a variety of qualitative and quantitative considerations ( cf. Tate , C. A. , Bick , R. J. , Chu , A. , Van Winkle , W. B. , and Entman , M. L. ( 1985 ) J. Biol .
	manualset3
261471	4	424118	15	NULL	NULL	NULL	NULL	Tate , C. A.	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on a variety of qualitative and quantitative considerations ( cf. Tate , C. A. , Bick , R. J. , Chu , A. , Van Winkle , W. B. , and Entman , M. L. ( 1985 ) J. Biol .
	manualset3
261472	5	424118	15	NULL	NULL	NULL	NULL	Bick , R. J.	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on a variety of qualitative and quantitative considerations ( cf. Tate , C. A. , Bick , R. J. , Chu , A. , Van Winkle , W. B. , and Entman , M. L. ( 1985 ) J. Biol .
	manualset3
261473	6	424118	15	NULL	NULL	NULL	NULL	Chu , A.	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on a variety of qualitative and quantitative considerations ( cf. Tate , C. A. , Bick , R. J. , Chu , A. , Van Winkle , W. B. , and Entman , M. L. ( 1985 ) J. Biol .
	manualset3
261474	7	424118	15	NULL	NULL	NULL	NULL	Van Winkle , W. B. 	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on a variety of qualitative and quantitative considerations ( cf. Tate , C. A. , Bick , R. J. , Chu , A. , Van Winkle , W. B. , and Entman , M. L. ( 1985 ) J. Biol .
	manualset3
261475	8	424118	15	NULL	NULL	NULL	NULL	Entman , M. L.	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on a variety of qualitative and quantitative considerations ( cf. Tate , C. A. , Bick , R. J. , Chu , A. , Van Winkle , W. B. , and Entman , M. L. ( 1985 ) J. Biol .
	manualset3
261476	9	424118	15	NULL	NULL	NULL	NULL	1985	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on a variety of qualitative and quantitative considerations ( cf. Tate , C. A. , Bick , R. J. , Chu , A. , Van Winkle , W. B. , and Entman , M. L. ( 1985 ) J. Biol .
	manualset3
261477	10	424118	15	NULL	NULL	NULL	NULL	J. Biol	Journal												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on a variety of qualitative and quantitative considerations ( cf. Tate , C. A. , Bick , R. J. , Chu , A. , Van Winkle , W. B. , and Entman , M. L. ( 1985 ) J. Biol .
	manualset3
261478	1	424119	15	NULL	NULL	NULL	NULL	analysis 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on an analysis by the International Commission on Radiological Protection , the deterministic radiation weighting factor for alpha particles appears to lie in the range of about 5-10 .
	manualset3
261556	2	424119	15	NULL	NULL	NULL	NULL	International Commission on Radiological Protection	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on an analysis by the International Commission on Radiological Protection , the deterministic radiation weighting factor for alpha particles appears to lie in the range of about 5-10 .
	manualset3
261557	3	424119	15	NULL	NULL	NULL	NULL	radiation weighting factor	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on an analysis by the International Commission on Radiological Protection , the deterministic radiation weighting factor for alpha particles appears to lie in the range of about 5-10 .
	manualset3
261558	4	424119	15	NULL	NULL	NULL	NULL	alpha particles	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on an analysis by the International Commission on Radiological Protection , the deterministic radiation weighting factor for alpha particles appears to lie in the range of about 5-10 .
	manualset3
261559	5	424119	15	NULL	NULL	NULL	NULL	range	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on an analysis by the International Commission on Radiological Protection , the deterministic radiation weighting factor for alpha particles appears to lie in the range of about 5-10 .
	manualset3
261560	6	424119	15	NULL	NULL	NULL	NULL	5-10	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on an analysis by the International Commission on Radiological Protection , the deterministic radiation weighting factor for alpha particles appears to lie in the range of about 5-10 .
	manualset3
261561	1	424120	15	NULL	NULL	NULL	NULL	analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on an analysis of the relationship between resistivity and temperature , the lamellar nano MgB ( 2 ) grains in the prepared sample possess better grain connectivity than the typical morphology of MgB ( 2 ) samples prepared by traditional high-temperature sintering .
	manualset3
261565	2	424120	15	NULL	NULL	NULL	NULL	relationship	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on an analysis of the relationship between resistivity and temperature , the lamellar nano MgB ( 2 ) grains in the prepared sample possess better grain connectivity than the typical morphology of MgB ( 2 ) samples prepared by traditional high-temperature sintering .
	manualset3
261566	3	424120	15	NULL	NULL	NULL	NULL	resistivity	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on an analysis of the relationship between resistivity and temperature , the lamellar nano MgB ( 2 ) grains in the prepared sample possess better grain connectivity than the typical morphology of MgB ( 2 ) samples prepared by traditional high-temperature sintering .
	manualset3
261567	4	424120	15	NULL	NULL	NULL	NULL	temperature	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on an analysis of the relationship between resistivity and temperature , the lamellar nano MgB ( 2 ) grains in the prepared sample possess better grain connectivity than the typical morphology of MgB ( 2 ) samples prepared by traditional high-temperature sintering .
	manualset3
261575	5	424120	15	NULL	NULL	NULL	NULL	nano MgB ( 2 ) grains 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on an analysis of the relationship between resistivity and temperature , the lamellar nano MgB ( 2 ) grains in the prepared sample possess better grain connectivity than the typical morphology of MgB ( 2 ) samples prepared by traditional high-temperature sintering .
	manualset3
261578	6	424120	15	NULL	NULL	NULL	NULL	sample	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on an analysis of the relationship between resistivity and temperature , the lamellar nano MgB ( 2 ) grains in the prepared sample possess better grain connectivity than the typical morphology of MgB ( 2 ) samples prepared by traditional high-temperature sintering .
	manualset3
261580	7	424120	15	NULL	NULL	NULL	NULL	grain connectivity	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on an analysis of the relationship between resistivity and temperature , the lamellar nano MgB ( 2 ) grains in the prepared sample possess better grain connectivity than the typical morphology of MgB ( 2 ) samples prepared by traditional high-temperature sintering .
	manualset3
261582	8	424120	15	NULL	NULL	NULL	NULL	morphology 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on an analysis of the relationship between resistivity and temperature , the lamellar nano MgB ( 2 ) grains in the prepared sample possess better grain connectivity than the typical morphology of MgB ( 2 ) samples prepared by traditional high-temperature sintering .
	manualset3
261583	9	424120	15	NULL	NULL	NULL	NULL	MgB ( 2 ) samples	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on an analysis of the relationship between resistivity and temperature , the lamellar nano MgB ( 2 ) grains in the prepared sample possess better grain connectivity than the typical morphology of MgB ( 2 ) samples prepared by traditional high-temperature sintering .
	manualset3
261586	10	424120	15	NULL	NULL	NULL	NULL	high-temperature sintering	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on an analysis of the relationship between resistivity and temperature , the lamellar nano MgB ( 2 ) grains in the prepared sample possess better grain connectivity than the typical morphology of MgB ( 2 ) samples prepared by traditional high-temperature sintering .
	manualset3
261591	1	424121	15	NULL	NULL	NULL	NULL	Experiment	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experiment compared between iodoxamidic acid and ioglycamic acid , in flasks drop by drop .
	manualset3
261593	2	424121	15	NULL	NULL	NULL	NULL	iodoxamidic acid	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experiment compared between iodoxamidic acid and ioglycamic acid , in flasks drop by drop .
	manualset3
261594	3	424121	15	NULL	NULL	NULL	NULL	ioglycamic acid	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experiment compared between iodoxamidic acid and ioglycamic acid , in flasks drop by drop .
	manualset3
261597	4	424121	15	NULL	NULL	NULL	NULL	flasks	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experiment compared between iodoxamidic acid and ioglycamic acid , in flasks drop by drop .
	manualset3
261598	5	424121	15	NULL	NULL	NULL	NULL	drop by drop	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experiment compared between iodoxamidic acid and ioglycamic acid , in flasks drop by drop .
	manualset3
261601	1	424122	15	NULL	NULL	NULL	NULL	empirical application	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on an empirical application of the CTC ( M-1 ) model , a complex simulation study was conducted to examine the sample size requirements of the robust weighted least squares mean - and variance-adjusted chi ( 2 ) test of model fit ( WLSMV estimator ) implemented in Mplus .
	manualset3
261603	2	424122	15	NULL	NULL	NULL	NULL	CTC ( M-1 ) model 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on an empirical application of the CTC ( M-1 ) model , a complex simulation study was conducted to examine the sample size requirements of the robust weighted least squares mean - and variance-adjusted chi ( 2 ) test of model fit ( WLSMV estimator ) implemented in Mplus .
	manualset3
261605	3	424122	15	NULL	NULL	NULL	NULL	complex simulation study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on an empirical application of the CTC ( M-1 ) model , a complex simulation study was conducted to examine the sample size requirements of the robust weighted least squares mean - and variance-adjusted chi ( 2 ) test of model fit ( WLSMV estimator ) implemented in Mplus .
	manualset3
261609	4	424122	15	NULL	NULL	NULL	NULL	sample size requirements 	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on an empirical application of the CTC ( M-1 ) model , a complex simulation study was conducted to examine the sample size requirements of the robust weighted least squares mean - and variance-adjusted chi ( 2 ) test of model fit ( WLSMV estimator ) implemented in Mplus .
	manualset3
261611	5	424122	15	NULL	NULL	NULL	NULL	robust weighted least squares mean	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on an empirical application of the CTC ( M-1 ) model , a complex simulation study was conducted to examine the sample size requirements of the robust weighted least squares mean - and variance-adjusted chi ( 2 ) test of model fit ( WLSMV estimator ) implemented in Mplus .
	manualset3
261613	6	424122	15	NULL	NULL	NULL	NULL	variance	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on an empirical application of the CTC ( M-1 ) model , a complex simulation study was conducted to examine the sample size requirements of the robust weighted least squares mean - and variance-adjusted chi ( 2 ) test of model fit ( WLSMV estimator ) implemented in Mplus .
	manualset3
261617	7	424122	15	NULL	NULL	NULL	NULL	chi ( 2 ) test of model	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on an empirical application of the CTC ( M-1 ) model , a complex simulation study was conducted to examine the sample size requirements of the robust weighted least squares mean - and variance-adjusted chi ( 2 ) test of model fit ( WLSMV estimator ) implemented in Mplus .
	manualset3
261627	8	424122	15	NULL	NULL	NULL	NULL	fit ( WLSMV estimator ) 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on an empirical application of the CTC ( M-1 ) model , a complex simulation study was conducted to examine the sample size requirements of the robust weighted least squares mean - and variance-adjusted chi ( 2 ) test of model fit ( WLSMV estimator ) implemented in Mplus .
	manualset3
261630	9	424122	15	NULL	NULL	NULL	NULL	Mplus	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on an empirical application of the CTC ( M-1 ) model , a complex simulation study was conducted to examine the sample size requirements of the robust weighted least squares mean - and variance-adjusted chi ( 2 ) test of model fit ( WLSMV estimator ) implemented in Mplus .
	manualset3
261637	1	424123	15	NULL	NULL	NULL	NULL	current data 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on current data on Na/H exchanger isoforms ( NHE-1 to 5 ) , NHE-3 is the likeliest candidate for the apical membrane isoform .
	manualset3
261639	2	424123	15	NULL	NULL	NULL	NULL	Na/H exchanger isoforms ( NHE-1 to 5 )	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on current data on Na/H exchanger isoforms ( NHE-1 to 5 ) , NHE-3 is the likeliest candidate for the apical membrane isoform .
	manualset3
261640	3	424123	15	NULL	NULL	NULL	NULL	NHE-3	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on current data on Na/H exchanger isoforms ( NHE-1 to 5 ) , NHE-3 is the likeliest candidate for the apical membrane isoform .
	manualset3
261641	4	424123	15	NULL	NULL	NULL	NULL	candidate	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on current data on Na/H exchanger isoforms ( NHE-1 to 5 ) , NHE-3 is the likeliest candidate for the apical membrane isoform .
	manualset3
261642	5	424123	15	NULL	NULL	NULL	NULL	apical membrane isoform	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on current data on Na/H exchanger isoforms ( NHE-1 to 5 ) , NHE-3 is the likeliest candidate for the apical membrane isoform .
	manualset3
261646	1	424124	15	NULL	NULL	NULL	NULL	experimental inspiratory driving pressure waveforms	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on experimental inspiratory driving pressure waveforms and active respiratory impedance data of anesthetized cats , we made model predictions of the factors that determine the immediate ( first loaded breath ) intrinsic ( i.e. , nonneural ) tidal volume compensation to added inspiratory elastic loads .
	manualset3
261649	2	424124	15	NULL	NULL	NULL	NULL	active respiratory impedance data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on experimental inspiratory driving pressure waveforms and active respiratory impedance data of anesthetized cats , we made model predictions of the factors that determine the immediate ( first loaded breath ) intrinsic ( i.e. , nonneural ) tidal volume compensation to added inspiratory elastic loads .
	manualset3
261650	3	424124	15	NULL	NULL	NULL	NULL	cats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on experimental inspiratory driving pressure waveforms and active respiratory impedance data of anesthetized cats , we made model predictions of the factors that determine the immediate ( first loaded breath ) intrinsic ( i.e. , nonneural ) tidal volume compensation to added inspiratory elastic loads .
	manualset3
261651	4	424124	15	NULL	NULL	NULL	NULL	model predictions	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on experimental inspiratory driving pressure waveforms and active respiratory impedance data of anesthetized cats , we made model predictions of the factors that determine the immediate ( first loaded breath ) intrinsic ( i.e. , nonneural ) tidal volume compensation to added inspiratory elastic loads .
	manualset3
261652	5	424124	15	NULL	NULL	NULL	NULL	factors	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on experimental inspiratory driving pressure waveforms and active respiratory impedance data of anesthetized cats , we made model predictions of the factors that determine the immediate ( first loaded breath ) intrinsic ( i.e. , nonneural ) tidal volume compensation to added inspiratory elastic loads .
	manualset3
261655	6	424124	15	NULL	NULL	NULL	NULL	immediate ( first loaded breath ) intrinsic ( i.e. , nonneural ) tidal volume	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on experimental inspiratory driving pressure waveforms and active respiratory impedance data of anesthetized cats , we made model predictions of the factors that determine the immediate ( first loaded breath ) intrinsic ( i.e. , nonneural ) tidal volume compensation to added inspiratory elastic loads .
	manualset3
261656	7	424124	15	NULL	NULL	NULL	NULL	compensation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on experimental inspiratory driving pressure waveforms and active respiratory impedance data of anesthetized cats , we made model predictions of the factors that determine the immediate ( first loaded breath ) intrinsic ( i.e. , nonneural ) tidal volume compensation to added inspiratory elastic loads .
	manualset3
261657	8	424124	15	NULL	NULL	NULL	NULL	inspiratory elastic loads	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on experimental inspiratory driving pressure waveforms and active respiratory impedance data of anesthetized cats , we made model predictions of the factors that determine the immediate ( first loaded breath ) intrinsic ( i.e. , nonneural ) tidal volume compensation to added inspiratory elastic loads .
	manualset3
261661	1	424125	15	NULL	NULL	NULL	NULL	extensive numerical simulations	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on extensive numerical simulations , it is shown that the interface width exhibits a growing regime that at time t ( x2 ) crosses over to a saturation state such that the width ( Wsat ) remains stationary .
	manualset3
261662	2	424125	15	NULL	NULL	NULL	NULL	interface width	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on extensive numerical simulations , it is shown that the interface width exhibits a growing regime that at time t ( x2 ) crosses over to a saturation state such that the width ( Wsat ) remains stationary .
	manualset3
261663	3	424125	15	NULL	NULL	NULL	NULL	growing regime	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on extensive numerical simulations , it is shown that the interface width exhibits a growing regime that at time t ( x2 ) crosses over to a saturation state such that the width ( Wsat ) remains stationary .
	manualset3
261665	4	424125	15	NULL	NULL	NULL	NULL	time t ( x2 ) 	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on extensive numerical simulations , it is shown that the interface width exhibits a growing regime that at time t ( x2 ) crosses over to a saturation state such that the width ( Wsat ) remains stationary .
	manualset3
261668	5	424125	15	NULL	NULL	NULL	NULL	saturation state	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on extensive numerical simulations , it is shown that the interface width exhibits a growing regime that at time t ( x2 ) crosses over to a saturation state such that the width ( Wsat ) remains stationary .
	manualset3
261670	6	424125	15	NULL	NULL	NULL	NULL	width ( Wsat )	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on extensive numerical simulations , it is shown that the interface width exhibits a growing regime that at time t ( x2 ) crosses over to a saturation state such that the width ( Wsat ) remains stationary .
	manualset3
261678	1	424126	15	NULL	NULL	NULL	NULL	family interaction theory	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on family interaction theory , the study examined the interrelationships among acculturation variables , family relationships , girls ' depressed mood , peer alcohol use , and girls ' alcohol use in a sample of 130 Asian American mother-daughter dyads .
	manualset3
261679	2	424126	15	NULL	NULL	NULL	NULL	study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on family interaction theory , the study examined the interrelationships among acculturation variables , family relationships , girls ' depressed mood , peer alcohol use , and girls ' alcohol use in a sample of 130 Asian American mother-daughter dyads .
	manualset3
261680	3	424126	15	NULL	NULL	NULL	NULL	interrelationships	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on family interaction theory , the study examined the interrelationships among acculturation variables , family relationships , girls ' depressed mood , peer alcohol use , and girls ' alcohol use in a sample of 130 Asian American mother-daughter dyads .
	manualset3
261682	4	424126	15	NULL	NULL	NULL	NULL	acculturation variables	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on family interaction theory , the study examined the interrelationships among acculturation variables , family relationships , girls ' depressed mood , peer alcohol use , and girls ' alcohol use in a sample of 130 Asian American mother-daughter dyads .
	manualset3
261683	5	424126	15	NULL	NULL	NULL	NULL	family relationships	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on family interaction theory , the study examined the interrelationships among acculturation variables , family relationships , girls ' depressed mood , peer alcohol use , and girls ' alcohol use in a sample of 130 Asian American mother-daughter dyads .
	manualset3
261685	6	424126	15	NULL	NULL	NULL	NULL	girls ' depressed mood 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on family interaction theory , the study examined the interrelationships among acculturation variables , family relationships , girls ' depressed mood , peer alcohol use , and girls ' alcohol use in a sample of 130 Asian American mother-daughter dyads .
	manualset3
261687	7	424126	15	NULL	NULL	NULL	NULL	peer alcohol use	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on family interaction theory , the study examined the interrelationships among acculturation variables , family relationships , girls ' depressed mood , peer alcohol use , and girls ' alcohol use in a sample of 130 Asian American mother-daughter dyads .
	manualset3
261689	8	424126	15	NULL	NULL	NULL	NULL	girls ' alcohol use	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on family interaction theory , the study examined the interrelationships among acculturation variables , family relationships , girls ' depressed mood , peer alcohol use , and girls ' alcohol use in a sample of 130 Asian American mother-daughter dyads .
	manualset3
261691	9	424126	15	NULL	NULL	NULL	NULL	sample 	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on family interaction theory , the study examined the interrelationships among acculturation variables , family relationships , girls ' depressed mood , peer alcohol use , and girls ' alcohol use in a sample of 130 Asian American mother-daughter dyads .
	manualset3
261693	10	424126	15	NULL	NULL	NULL	NULL	130	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on family interaction theory , the study examined the interrelationships among acculturation variables , family relationships , girls ' depressed mood , peer alcohol use , and girls ' alcohol use in a sample of 130 Asian American mother-daughter dyads .
	manualset3
261694	11	424126	15	NULL	NULL	NULL	NULL	Asian American mother-daughter dyads	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on family interaction theory , the study examined the interrelationships among acculturation variables , family relationships , girls ' depressed mood , peer alcohol use , and girls ' alcohol use in a sample of 130 Asian American mother-daughter dyads .
	manualset3
261702	1	424127	15	NULL	NULL	NULL	NULL	feedback 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on feedback obtained through a national program of heart failure workshops during 2006 and 2007 , several topics were identified as priorities because of the challenges they pose to health care professionals .
	manualset3
261704	2	424127	15	NULL	NULL	NULL	NULL	national program of heart failure workshops	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on feedback obtained through a national program of heart failure workshops during 2006 and 2007 , several topics were identified as priorities because of the challenges they pose to health care professionals .
	manualset3
261708	3	424127	15	NULL	NULL	NULL	NULL	2006	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on feedback obtained through a national program of heart failure workshops during 2006 and 2007 , several topics were identified as priorities because of the challenges they pose to health care professionals .
	manualset3
261711	4	424127	15	NULL	NULL	NULL	NULL	2007	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on feedback obtained through a national program of heart failure workshops during 2006 and 2007 , several topics were identified as priorities because of the challenges they pose to health care professionals .
	manualset3
261713	5	424127	15	NULL	NULL	NULL	NULL	topics	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on feedback obtained through a national program of heart failure workshops during 2006 and 2007 , several topics were identified as priorities because of the challenges they pose to health care professionals .
	manualset3
261714	6	424127	15	NULL	NULL	NULL	NULL	priorities	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on feedback obtained through a national program of heart failure workshops during 2006 and 2007 , several topics were identified as priorities because of the challenges they pose to health care professionals .
	manualset3
261715	7	424127	15	NULL	NULL	NULL	NULL	challenges	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on feedback obtained through a national program of heart failure workshops during 2006 and 2007 , several topics were identified as priorities because of the challenges they pose to health care professionals .
	manualset3
261718	8	424127	15	NULL	NULL	NULL	NULL	health care professionals	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on feedback obtained through a national program of heart failure workshops during 2006 and 2007 , several topics were identified as priorities because of the challenges they pose to health care professionals .
	manualset3
261737	1	424128	15	NULL	NULL	NULL	NULL	gene homology	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on gene homology , structure , and expression patterns , these findings indicate that mouse Ovca1 is the orthologue of human OVCA1/DPH2L1 .
	manualset3
261739	2	424128	15	NULL	NULL	NULL	NULL	structure 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on gene homology , structure , and expression patterns , these findings indicate that mouse Ovca1 is the orthologue of human OVCA1/DPH2L1 .
	manualset3
261742	3	424128	15	NULL	NULL	NULL	NULL	expression patterns	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on gene homology , structure , and expression patterns , these findings indicate that mouse Ovca1 is the orthologue of human OVCA1/DPH2L1 .
	manualset3
261744	4	424128	15	NULL	NULL	NULL	NULL	findings	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on gene homology , structure , and expression patterns , these findings indicate that mouse Ovca1 is the orthologue of human OVCA1/DPH2L1 .
	manualset3
261766	5	424128	15	NULL	NULL	NULL	NULL	mouse Ovca1	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on gene homology , structure , and expression patterns , these findings indicate that mouse Ovca1 is the orthologue of human OVCA1/DPH2L1 .
	manualset3
261767	6	424128	15	NULL	NULL	NULL	NULL	orthologue	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on gene homology , structure , and expression patterns , these findings indicate that mouse Ovca1 is the orthologue of human OVCA1/DPH2L1 .
	manualset3
261768	7	424128	15	NULL	NULL	NULL	NULL	human OVCA1/DPH2L1	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on gene homology , structure , and expression patterns , these findings indicate that mouse Ovca1 is the orthologue of human OVCA1/DPH2L1 .
	manualset3
261769	1	424129	15	NULL	NULL	NULL	NULL	histochemical analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on histochemical analysis of oxalate-deficient and wild-type strains of S. sclerotiorum , oxalate caused a decrease in hydrogen peroxide production but no detectable changes in plant superoxide production or gene expression .
	manualset3
261770	2	424129	15	NULL	NULL	NULL	NULL	oxalate-deficient strains 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on histochemical analysis of oxalate-deficient and wild-type strains of S. sclerotiorum , oxalate caused a decrease in hydrogen peroxide production but no detectable changes in plant superoxide production or gene expression .
	manualset3
261771	3	424129	15	NULL	NULL	NULL	NULL	wild-type strains	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on histochemical analysis of oxalate-deficient and wild-type strains of S. sclerotiorum , oxalate caused a decrease in hydrogen peroxide production but no detectable changes in plant superoxide production or gene expression .
	manualset3
261772	4	424129	15	NULL	NULL	NULL	NULL	S. sclerotiorum	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on histochemical analysis of oxalate-deficient and wild-type strains of S. sclerotiorum , oxalate caused a decrease in hydrogen peroxide production but no detectable changes in plant superoxide production or gene expression .
	manualset3
261773	5	424129	15	NULL	NULL	NULL	NULL	oxalate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on histochemical analysis of oxalate-deficient and wild-type strains of S. sclerotiorum , oxalate caused a decrease in hydrogen peroxide production but no detectable changes in plant superoxide production or gene expression .
	manualset3
261774	6	424129	15	NULL	NULL	NULL	NULL	decrease	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on histochemical analysis of oxalate-deficient and wild-type strains of S. sclerotiorum , oxalate caused a decrease in hydrogen peroxide production but no detectable changes in plant superoxide production or gene expression .
	manualset3
261775	7	424129	15	NULL	NULL	NULL	NULL	hydrogen peroxide production	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on histochemical analysis of oxalate-deficient and wild-type strains of S. sclerotiorum , oxalate caused a decrease in hydrogen peroxide production but no detectable changes in plant superoxide production or gene expression .
	manualset3
261776	8	424129	15	NULL	NULL	NULL	NULL	changes	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on histochemical analysis of oxalate-deficient and wild-type strains of S. sclerotiorum , oxalate caused a decrease in hydrogen peroxide production but no detectable changes in plant superoxide production or gene expression .
	manualset3
261777	9	424129	15	NULL	NULL	NULL	NULL	plant superoxide production	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on histochemical analysis of oxalate-deficient and wild-type strains of S. sclerotiorum , oxalate caused a decrease in hydrogen peroxide production but no detectable changes in plant superoxide production or gene expression .
	manualset3
261778	10	424129	15	NULL	NULL	NULL	NULL	gene expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on histochemical analysis of oxalate-deficient and wild-type strains of S. sclerotiorum , oxalate caused a decrease in hydrogen peroxide production but no detectable changes in plant superoxide production or gene expression .
	manualset3
261779	1	424130	15	NULL	NULL	NULL	NULL	Experimental studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental and clinical studies on tubazine ) .
	manualset3
261780	2	424130	15	NULL	NULL	NULL	NULL	clinical studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental and clinical studies on tubazine ) .
	manualset3
261781	3	424130	15	NULL	NULL	NULL	NULL	tubazine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental and clinical studies on tubazine ) .
	manualset3
261782	1	424131	15	NULL	NULL	NULL	NULL	multivariate analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on multivariate analysis , factors associated with not having Pap smears were : age ( 40-59 years ) , race/ethnicity ( black or mixed-race ) , and schooling ( & lt ; 4 years ) .
	manualset3
261783	2	424131	15	NULL	NULL	NULL	NULL	factors	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on multivariate analysis , factors associated with not having Pap smears were : age ( 40-59 years ) , race/ethnicity ( black or mixed-race ) , and schooling ( & lt ; 4 years ) .
	manualset3
261784	3	424131	15	NULL	NULL	NULL	NULL	Pap smears	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on multivariate analysis , factors associated with not having Pap smears were : age ( 40-59 years ) , race/ethnicity ( black or mixed-race ) , and schooling ( & lt ; 4 years ) .
	manualset3
261785	4	424131	15	NULL	NULL	NULL	NULL	age ( 40-59 years )	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on multivariate analysis , factors associated with not having Pap smears were : age ( 40-59 years ) , race/ethnicity ( black or mixed-race ) , and schooling ( & lt ; 4 years ) .
	manualset3
261786	5	424131	15	NULL	NULL	NULL	NULL	race/ethnicity ( black or mixed-race ) 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on multivariate analysis , factors associated with not having Pap smears were : age ( 40-59 years ) , race/ethnicity ( black or mixed-race ) , and schooling ( & lt ; 4 years ) .
	manualset3
261787	6	424131	15	NULL	NULL	NULL	NULL	schooling 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on multivariate analysis , factors associated with not having Pap smears were : age ( 40-59 years ) , race/ethnicity ( black or mixed-race ) , and schooling ( & lt ; 4 years ) .
	manualset3
261788	7	424131	15	NULL	NULL	NULL	NULL	& lt ; 4 years	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on multivariate analysis , factors associated with not having Pap smears were : age ( 40-59 years ) , race/ethnicity ( black or mixed-race ) , and schooling ( & lt ; 4 years ) .
	manualset3
261789	1	424132	15	NULL	NULL	NULL	NULL	initial experience 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on our initial experience , laparoscopic colposuspension appears to be a viable alternative to abdominal colposuspension .
	manualset3
261790	2	424132	15	NULL	NULL	NULL	NULL	laparoscopic colposuspension	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on our initial experience , laparoscopic colposuspension appears to be a viable alternative to abdominal colposuspension .
	manualset3
261791	3	424132	15	NULL	NULL	NULL	NULL	abdominal colposuspension 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on our initial experience , laparoscopic colposuspension appears to be a viable alternative to abdominal colposuspension .
	manualset3
261792	1	424133	15	NULL	NULL	NULL	NULL	observations	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on our observations on the biology of both structural and regulatory genes of the nitrogen assimilatory pathway , we have developed a model for metabolic control of the genes involved in the nitrogen assimilatory pathway in plants .
	manualset3
261793	2	424133	15	NULL	NULL	NULL	NULL	biology	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on our observations on the biology of both structural and regulatory genes of the nitrogen assimilatory pathway , we have developed a model for metabolic control of the genes involved in the nitrogen assimilatory pathway in plants .
	manualset3
261794	3	424133	15	NULL	NULL	NULL	NULL	structural genes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on our observations on the biology of both structural and regulatory genes of the nitrogen assimilatory pathway , we have developed a model for metabolic control of the genes involved in the nitrogen assimilatory pathway in plants .
	manualset3
261795	4	424133	15	NULL	NULL	NULL	NULL	regulatory genes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on our observations on the biology of both structural and regulatory genes of the nitrogen assimilatory pathway , we have developed a model for metabolic control of the genes involved in the nitrogen assimilatory pathway in plants .
	manualset3
261796	5	424133	15	NULL	NULL	NULL	NULL	nitrogen assimilatory pathway	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on our observations on the biology of both structural and regulatory genes of the nitrogen assimilatory pathway , we have developed a model for metabolic control of the genes involved in the nitrogen assimilatory pathway in plants .
	manualset3
261797	6	424133	15	NULL	NULL	NULL	NULL	model	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on our observations on the biology of both structural and regulatory genes of the nitrogen assimilatory pathway , we have developed a model for metabolic control of the genes involved in the nitrogen assimilatory pathway in plants .
	manualset3
261798	7	424133	15	NULL	NULL	NULL	NULL	metabolic control of the genes	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on our observations on the biology of both structural and regulatory genes of the nitrogen assimilatory pathway , we have developed a model for metabolic control of the genes involved in the nitrogen assimilatory pathway in plants .
	manualset3
261799	8	424133	15	NULL	NULL	NULL	NULL	nitrogen assimilatory pathway	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on our observations on the biology of both structural and regulatory genes of the nitrogen assimilatory pathway , we have developed a model for metabolic control of the genes involved in the nitrogen assimilatory pathway in plants .
	manualset3
261800	9	424133	15	NULL	NULL	NULL	NULL	plants	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on our observations on the biology of both structural and regulatory genes of the nitrogen assimilatory pathway , we have developed a model for metabolic control of the genes involved in the nitrogen assimilatory pathway in plants .
	manualset3
261801	1	424134	15	NULL	NULL	NULL	NULL	results	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on our results , continuous production of 1 , 3-PDO with immobilized cells is an efficient method , and raw glycerol can be utilized without any pretreatment .
	manualset3
261802	2	424134	15	NULL	NULL	NULL	NULL	production of 1 , 3-PDO	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on our results , continuous production of 1 , 3-PDO with immobilized cells is an efficient method , and raw glycerol can be utilized without any pretreatment .
	manualset3
261803	3	424134	15	NULL	NULL	NULL	NULL	immobilized cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on our results , continuous production of 1 , 3-PDO with immobilized cells is an efficient method , and raw glycerol can be utilized without any pretreatment .
	manualset3
261804	4	424134	15	NULL	NULL	NULL	NULL	efficient method	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on our results , continuous production of 1 , 3-PDO with immobilized cells is an efficient method , and raw glycerol can be utilized without any pretreatment .
	manualset3
261805	5	424134	15	NULL	NULL	NULL	NULL	raw glycerol 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on our results , continuous production of 1 , 3-PDO with immobilized cells is an efficient method , and raw glycerol can be utilized without any pretreatment .
	manualset3
261806	6	424134	15	NULL	NULL	NULL	NULL	pretreatment 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on our results , continuous production of 1 , 3-PDO with immobilized cells is an efficient method , and raw glycerol can be utilized without any pretreatment .
	manualset3
261807	1	424135	15	NULL	NULL	NULL	NULL	partial amino acid sequences	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on partial amino acid sequences of rat p144 , mouse p144 cDNA was cloned and sequenced , and its amino acid sequence was predicted .
	manualset3
261808	2	424135	15	NULL	NULL	NULL	NULL	rat p144	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on partial amino acid sequences of rat p144 , mouse p144 cDNA was cloned and sequenced , and its amino acid sequence was predicted .
	manualset3
261809	3	424135	15	NULL	NULL	NULL	NULL	mouse p144 cDNA	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on partial amino acid sequences of rat p144 , mouse p144 cDNA was cloned and sequenced , and its amino acid sequence was predicted .
	manualset3
261810	4	424135	15	NULL	NULL	NULL	NULL	amino acid sequence	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on partial amino acid sequences of rat p144 , mouse p144 cDNA was cloned and sequenced , and its amino acid sequence was predicted .
	manualset3
261811	1	424136	15	NULL	NULL	NULL	NULL	pathogenesis studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on pathogenesis studies MHV strains are usually grouped according to their primary tissue tropism into two biotypes : polytropic and enterotropic .
	manualset3
261812	2	424136	15	NULL	NULL	NULL	NULL	MHV strains	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on pathogenesis studies MHV strains are usually grouped according to their primary tissue tropism into two biotypes : polytropic and enterotropic .
	manualset3
261813	3	424136	15	NULL	NULL	NULL	NULL	primary tissue tropism	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on pathogenesis studies MHV strains are usually grouped according to their primary tissue tropism into two biotypes : polytropic and enterotropic .
	manualset3
261814	4	424136	15	NULL	NULL	NULL	NULL	two biotypes 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on pathogenesis studies MHV strains are usually grouped according to their primary tissue tropism into two biotypes : polytropic and enterotropic .
	manualset3
261815	5	424136	15	NULL	NULL	NULL	NULL	polytropic	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on pathogenesis studies MHV strains are usually grouped according to their primary tissue tropism into two biotypes : polytropic and enterotropic .
	manualset3
261816	6	424136	15	NULL	NULL	NULL	NULL	enterotropic	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on pathogenesis studies MHV strains are usually grouped according to their primary tissue tropism into two biotypes : polytropic and enterotropic .
	manualset3
261817	1	424137	15	NULL	NULL	NULL	NULL	recent evidence	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on recent evidence that fatty acid synthase and endogenously produced fatty acid derivatives are required for adipogenesis in 3T3-L1 adipocytes , we conducted a small interfering RNA-based screen to identify other fatty acid-metabolizing enzymes that may mediate this effect .
	manualset3
261818	2	424137	15	NULL	NULL	NULL	NULL	fatty acid synthase	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on recent evidence that fatty acid synthase and endogenously produced fatty acid derivatives are required for adipogenesis in 3T3-L1 adipocytes , we conducted a small interfering RNA-based screen to identify other fatty acid-metabolizing enzymes that may mediate this effect .
	manualset3
261819	3	424137	15	NULL	NULL	NULL	NULL	fatty acid derivatives	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on recent evidence that fatty acid synthase and endogenously produced fatty acid derivatives are required for adipogenesis in 3T3-L1 adipocytes , we conducted a small interfering RNA-based screen to identify other fatty acid-metabolizing enzymes that may mediate this effect .
	manualset3
261820	4	424137	15	NULL	NULL	NULL	NULL	adipogenesis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on recent evidence that fatty acid synthase and endogenously produced fatty acid derivatives are required for adipogenesis in 3T3-L1 adipocytes , we conducted a small interfering RNA-based screen to identify other fatty acid-metabolizing enzymes that may mediate this effect .
	manualset3
261821	5	424137	15	NULL	NULL	NULL	NULL	3T3-L1 adipocytes 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on recent evidence that fatty acid synthase and endogenously produced fatty acid derivatives are required for adipogenesis in 3T3-L1 adipocytes , we conducted a small interfering RNA-based screen to identify other fatty acid-metabolizing enzymes that may mediate this effect .
	manualset3
261822	6	424137	15	NULL	NULL	NULL	NULL	small interfering RNA-based screen	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on recent evidence that fatty acid synthase and endogenously produced fatty acid derivatives are required for adipogenesis in 3T3-L1 adipocytes , we conducted a small interfering RNA-based screen to identify other fatty acid-metabolizing enzymes that may mediate this effect .
	manualset3
261823	7	424137	15	NULL	NULL	NULL	NULL	fatty acid-metabolizing enzymes 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on recent evidence that fatty acid synthase and endogenously produced fatty acid derivatives are required for adipogenesis in 3T3-L1 adipocytes , we conducted a small interfering RNA-based screen to identify other fatty acid-metabolizing enzymes that may mediate this effect .
	manualset3
261824	8	424137	15	NULL	NULL	NULL	NULL	effect	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on recent evidence that fatty acid synthase and endogenously produced fatty acid derivatives are required for adipogenesis in 3T3-L1 adipocytes , we conducted a small interfering RNA-based screen to identify other fatty acid-metabolizing enzymes that may mediate this effect .
	manualset3
261825	1	424138	15	NULL	NULL	NULL	NULL	cDNA structure	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the cDNA structure and the known amino acid sequence of the mature peptide , it was concluded that the precursor of halocidin contains a 21-residue signal peptide , followed by the 18 residues of the mature peptide , and a 56-residue anionic C-terminal extension , which is removed later on in the process .
	manualset3
261826	2	424138	15	NULL	NULL	NULL	NULL	amino acid sequence	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the cDNA structure and the known amino acid sequence of the mature peptide , it was concluded that the precursor of halocidin contains a 21-residue signal peptide , followed by the 18 residues of the mature peptide , and a 56-residue anionic C-terminal extension , which is removed later on in the process .
	manualset3
261827	3	424138	15	NULL	NULL	NULL	NULL	mature peptide	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the cDNA structure and the known amino acid sequence of the mature peptide , it was concluded that the precursor of halocidin contains a 21-residue signal peptide , followed by the 18 residues of the mature peptide , and a 56-residue anionic C-terminal extension , which is removed later on in the process .
	manualset3
261828	4	424138	15	NULL	NULL	NULL	NULL	precursor	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the cDNA structure and the known amino acid sequence of the mature peptide , it was concluded that the precursor of halocidin contains a 21-residue signal peptide , followed by the 18 residues of the mature peptide , and a 56-residue anionic C-terminal extension , which is removed later on in the process .
	manualset3
261829	5	424138	15	NULL	NULL	NULL	NULL	halocidin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the cDNA structure and the known amino acid sequence of the mature peptide , it was concluded that the precursor of halocidin contains a 21-residue signal peptide , followed by the 18 residues of the mature peptide , and a 56-residue anionic C-terminal extension , which is removed later on in the process .
	manualset3
261830	6	424138	15	NULL	NULL	NULL	NULL	21-residue	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the cDNA structure and the known amino acid sequence of the mature peptide , it was concluded that the precursor of halocidin contains a 21-residue signal peptide , followed by the 18 residues of the mature peptide , and a 56-residue anionic C-terminal extension , which is removed later on in the process .
	manualset3
261831	7	424138	15	NULL	NULL	NULL	NULL	signal peptide	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the cDNA structure and the known amino acid sequence of the mature peptide , it was concluded that the precursor of halocidin contains a 21-residue signal peptide , followed by the 18 residues of the mature peptide , and a 56-residue anionic C-terminal extension , which is removed later on in the process .
	manualset3
261832	8	424138	15	NULL	NULL	NULL	NULL	18 residues	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the cDNA structure and the known amino acid sequence of the mature peptide , it was concluded that the precursor of halocidin contains a 21-residue signal peptide , followed by the 18 residues of the mature peptide , and a 56-residue anionic C-terminal extension , which is removed later on in the process .
	manualset3
261833	9	424138	15	NULL	NULL	NULL	NULL	mature peptide	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the cDNA structure and the known amino acid sequence of the mature peptide , it was concluded that the precursor of halocidin contains a 21-residue signal peptide , followed by the 18 residues of the mature peptide , and a 56-residue anionic C-terminal extension , which is removed later on in the process .
	manualset3
261834	10	424138	15	NULL	NULL	NULL	NULL	56-residue	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the cDNA structure and the known amino acid sequence of the mature peptide , it was concluded that the precursor of halocidin contains a 21-residue signal peptide , followed by the 18 residues of the mature peptide , and a 56-residue anionic C-terminal extension , which is removed later on in the process .
	manualset3
261835	11	424138	15	NULL	NULL	NULL	NULL	anionic C-terminal extension	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the cDNA structure and the known amino acid sequence of the mature peptide , it was concluded that the precursor of halocidin contains a 21-residue signal peptide , followed by the 18 residues of the mature peptide , and a 56-residue anionic C-terminal extension , which is removed later on in the process .
	manualset3
261836	12	424138	15	NULL	NULL	NULL	NULL	process 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the cDNA structure and the known amino acid sequence of the mature peptide , it was concluded that the precursor of halocidin contains a 21-residue signal peptide , followed by the 18 residues of the mature peptide , and a 56-residue anionic C-terminal extension , which is removed later on in the process .
	manualset3
261837	1	424139	15	NULL	NULL	NULL	NULL	computational analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the computational analysis , it is found that ( 1 ) recruitment to membranes is facilitated by non-specific electrostatic interactions that occur between basic residues on the domains and acidic phospholipids in the membrane , ( 2 ) the energetic analysis can quantitatively differentiate among the modes of membrane association proposed by the experimentally determined structures , ( 3 ) FDPB calculations predict energetically feasible models for the membrane-associated states of FYVE domains , ( 4 ) these models are consistent with the observation that conserved hydrophobic residues insert into the membrane interface , and ( 5 ) the calculations provide a molecular model for the hydrophobic partitioning : binding of PI ( 3 ) P significantly neutralizes positive potential in the region of the hydrophobic residues , which acts as an `` electrostatic switch '' by reducing the energetic barrier for membrane penetration .
	manualset3
261838	2	424139	15	NULL	NULL	NULL	NULL	recruitment to membranes	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the computational analysis , it is found that ( 1 ) recruitment to membranes is facilitated by non-specific electrostatic interactions that occur between basic residues on the domains and acidic phospholipids in the membrane , ( 2 ) the energetic analysis can quantitatively differentiate among the modes of membrane association proposed by the experimentally determined structures , ( 3 ) FDPB calculations predict energetically feasible models for the membrane-associated states of FYVE domains , ( 4 ) these models are consistent with the observation that conserved hydrophobic residues insert into the membrane interface , and ( 5 ) the calculations provide a molecular model for the hydrophobic partitioning : binding of PI ( 3 ) P significantly neutralizes positive potential in the region of the hydrophobic residues , which acts as an `` electrostatic switch '' by reducing the energetic barrier for membrane penetration .
	manualset3
261839	3	424139	15	NULL	NULL	NULL	NULL	non-specific electrostatic interactions	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the computational analysis , it is found that ( 1 ) recruitment to membranes is facilitated by non-specific electrostatic interactions that occur between basic residues on the domains and acidic phospholipids in the membrane , ( 2 ) the energetic analysis can quantitatively differentiate among the modes of membrane association proposed by the experimentally determined structures , ( 3 ) FDPB calculations predict energetically feasible models for the membrane-associated states of FYVE domains , ( 4 ) these models are consistent with the observation that conserved hydrophobic residues insert into the membrane interface , and ( 5 ) the calculations provide a molecular model for the hydrophobic partitioning : binding of PI ( 3 ) P significantly neutralizes positive potential in the region of the hydrophobic residues , which acts as an `` electrostatic switch '' by reducing the energetic barrier for membrane penetration .
	manualset3
261840	4	424139	15	NULL	NULL	NULL	NULL	basic residues	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the computational analysis , it is found that ( 1 ) recruitment to membranes is facilitated by non-specific electrostatic interactions that occur between basic residues on the domains and acidic phospholipids in the membrane , ( 2 ) the energetic analysis can quantitatively differentiate among the modes of membrane association proposed by the experimentally determined structures , ( 3 ) FDPB calculations predict energetically feasible models for the membrane-associated states of FYVE domains , ( 4 ) these models are consistent with the observation that conserved hydrophobic residues insert into the membrane interface , and ( 5 ) the calculations provide a molecular model for the hydrophobic partitioning : binding of PI ( 3 ) P significantly neutralizes positive potential in the region of the hydrophobic residues , which acts as an `` electrostatic switch '' by reducing the energetic barrier for membrane penetration .
	manualset3
261841	5	424139	15	NULL	NULL	NULL	NULL	domains	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the computational analysis , it is found that ( 1 ) recruitment to membranes is facilitated by non-specific electrostatic interactions that occur between basic residues on the domains and acidic phospholipids in the membrane , ( 2 ) the energetic analysis can quantitatively differentiate among the modes of membrane association proposed by the experimentally determined structures , ( 3 ) FDPB calculations predict energetically feasible models for the membrane-associated states of FYVE domains , ( 4 ) these models are consistent with the observation that conserved hydrophobic residues insert into the membrane interface , and ( 5 ) the calculations provide a molecular model for the hydrophobic partitioning : binding of PI ( 3 ) P significantly neutralizes positive potential in the region of the hydrophobic residues , which acts as an `` electrostatic switch '' by reducing the energetic barrier for membrane penetration .
	manualset3
261842	6	424139	15	NULL	NULL	NULL	NULL	acidic phospholipids	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the computational analysis , it is found that ( 1 ) recruitment to membranes is facilitated by non-specific electrostatic interactions that occur between basic residues on the domains and acidic phospholipids in the membrane , ( 2 ) the energetic analysis can quantitatively differentiate among the modes of membrane association proposed by the experimentally determined structures , ( 3 ) FDPB calculations predict energetically feasible models for the membrane-associated states of FYVE domains , ( 4 ) these models are consistent with the observation that conserved hydrophobic residues insert into the membrane interface , and ( 5 ) the calculations provide a molecular model for the hydrophobic partitioning : binding of PI ( 3 ) P significantly neutralizes positive potential in the region of the hydrophobic residues , which acts as an `` electrostatic switch '' by reducing the energetic barrier for membrane penetration .
	manualset3
261843	7	424139	15	NULL	NULL	NULL	NULL	membrane	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the computational analysis , it is found that ( 1 ) recruitment to membranes is facilitated by non-specific electrostatic interactions that occur between basic residues on the domains and acidic phospholipids in the membrane , ( 2 ) the energetic analysis can quantitatively differentiate among the modes of membrane association proposed by the experimentally determined structures , ( 3 ) FDPB calculations predict energetically feasible models for the membrane-associated states of FYVE domains , ( 4 ) these models are consistent with the observation that conserved hydrophobic residues insert into the membrane interface , and ( 5 ) the calculations provide a molecular model for the hydrophobic partitioning : binding of PI ( 3 ) P significantly neutralizes positive potential in the region of the hydrophobic residues , which acts as an `` electrostatic switch '' by reducing the energetic barrier for membrane penetration .
	manualset3
261844	8	424139	15	NULL	NULL	NULL	NULL	energetic analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the computational analysis , it is found that ( 1 ) recruitment to membranes is facilitated by non-specific electrostatic interactions that occur between basic residues on the domains and acidic phospholipids in the membrane , ( 2 ) the energetic analysis can quantitatively differentiate among the modes of membrane association proposed by the experimentally determined structures , ( 3 ) FDPB calculations predict energetically feasible models for the membrane-associated states of FYVE domains , ( 4 ) these models are consistent with the observation that conserved hydrophobic residues insert into the membrane interface , and ( 5 ) the calculations provide a molecular model for the hydrophobic partitioning : binding of PI ( 3 ) P significantly neutralizes positive potential in the region of the hydrophobic residues , which acts as an `` electrostatic switch '' by reducing the energetic barrier for membrane penetration .
	manualset3
261845	9	424139	15	NULL	NULL	NULL	NULL	modes of membrane association	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the computational analysis , it is found that ( 1 ) recruitment to membranes is facilitated by non-specific electrostatic interactions that occur between basic residues on the domains and acidic phospholipids in the membrane , ( 2 ) the energetic analysis can quantitatively differentiate among the modes of membrane association proposed by the experimentally determined structures , ( 3 ) FDPB calculations predict energetically feasible models for the membrane-associated states of FYVE domains , ( 4 ) these models are consistent with the observation that conserved hydrophobic residues insert into the membrane interface , and ( 5 ) the calculations provide a molecular model for the hydrophobic partitioning : binding of PI ( 3 ) P significantly neutralizes positive potential in the region of the hydrophobic residues , which acts as an `` electrostatic switch '' by reducing the energetic barrier for membrane penetration .
	manualset3
261846	10	424139	15	NULL	NULL	NULL	NULL	structures	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the computational analysis , it is found that ( 1 ) recruitment to membranes is facilitated by non-specific electrostatic interactions that occur between basic residues on the domains and acidic phospholipids in the membrane , ( 2 ) the energetic analysis can quantitatively differentiate among the modes of membrane association proposed by the experimentally determined structures , ( 3 ) FDPB calculations predict energetically feasible models for the membrane-associated states of FYVE domains , ( 4 ) these models are consistent with the observation that conserved hydrophobic residues insert into the membrane interface , and ( 5 ) the calculations provide a molecular model for the hydrophobic partitioning : binding of PI ( 3 ) P significantly neutralizes positive potential in the region of the hydrophobic residues , which acts as an `` electrostatic switch '' by reducing the energetic barrier for membrane penetration .
	manualset3
261848	11	424139	15	NULL	NULL	NULL	NULL	( 3 ) FDPB calculations	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the computational analysis , it is found that ( 1 ) recruitment to membranes is facilitated by non-specific electrostatic interactions that occur between basic residues on the domains and acidic phospholipids in the membrane , ( 2 ) the energetic analysis can quantitatively differentiate among the modes of membrane association proposed by the experimentally determined structures , ( 3 ) FDPB calculations predict energetically feasible models for the membrane-associated states of FYVE domains , ( 4 ) these models are consistent with the observation that conserved hydrophobic residues insert into the membrane interface , and ( 5 ) the calculations provide a molecular model for the hydrophobic partitioning : binding of PI ( 3 ) P significantly neutralizes positive potential in the region of the hydrophobic residues , which acts as an `` electrostatic switch '' by reducing the energetic barrier for membrane penetration .
	manualset3
261849	12	424139	15	NULL	NULL	NULL	NULL	energetically feasible models	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the computational analysis , it is found that ( 1 ) recruitment to membranes is facilitated by non-specific electrostatic interactions that occur between basic residues on the domains and acidic phospholipids in the membrane , ( 2 ) the energetic analysis can quantitatively differentiate among the modes of membrane association proposed by the experimentally determined structures , ( 3 ) FDPB calculations predict energetically feasible models for the membrane-associated states of FYVE domains , ( 4 ) these models are consistent with the observation that conserved hydrophobic residues insert into the membrane interface , and ( 5 ) the calculations provide a molecular model for the hydrophobic partitioning : binding of PI ( 3 ) P significantly neutralizes positive potential in the region of the hydrophobic residues , which acts as an `` electrostatic switch '' by reducing the energetic barrier for membrane penetration .
	manualset3
261850	13	424139	15	NULL	NULL	NULL	NULL	membrane-associated states 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the computational analysis , it is found that ( 1 ) recruitment to membranes is facilitated by non-specific electrostatic interactions that occur between basic residues on the domains and acidic phospholipids in the membrane , ( 2 ) the energetic analysis can quantitatively differentiate among the modes of membrane association proposed by the experimentally determined structures , ( 3 ) FDPB calculations predict energetically feasible models for the membrane-associated states of FYVE domains , ( 4 ) these models are consistent with the observation that conserved hydrophobic residues insert into the membrane interface , and ( 5 ) the calculations provide a molecular model for the hydrophobic partitioning : binding of PI ( 3 ) P significantly neutralizes positive potential in the region of the hydrophobic residues , which acts as an `` electrostatic switch '' by reducing the energetic barrier for membrane penetration .
	manualset3
261851	14	424139	15	NULL	NULL	NULL	NULL	FYVE domains	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the computational analysis , it is found that ( 1 ) recruitment to membranes is facilitated by non-specific electrostatic interactions that occur between basic residues on the domains and acidic phospholipids in the membrane , ( 2 ) the energetic analysis can quantitatively differentiate among the modes of membrane association proposed by the experimentally determined structures , ( 3 ) FDPB calculations predict energetically feasible models for the membrane-associated states of FYVE domains , ( 4 ) these models are consistent with the observation that conserved hydrophobic residues insert into the membrane interface , and ( 5 ) the calculations provide a molecular model for the hydrophobic partitioning : binding of PI ( 3 ) P significantly neutralizes positive potential in the region of the hydrophobic residues , which acts as an `` electrostatic switch '' by reducing the energetic barrier for membrane penetration .
	manualset3
261852	15	424139	15	NULL	NULL	NULL	NULL	models 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the computational analysis , it is found that ( 1 ) recruitment to membranes is facilitated by non-specific electrostatic interactions that occur between basic residues on the domains and acidic phospholipids in the membrane , ( 2 ) the energetic analysis can quantitatively differentiate among the modes of membrane association proposed by the experimentally determined structures , ( 3 ) FDPB calculations predict energetically feasible models for the membrane-associated states of FYVE domains , ( 4 ) these models are consistent with the observation that conserved hydrophobic residues insert into the membrane interface , and ( 5 ) the calculations provide a molecular model for the hydrophobic partitioning : binding of PI ( 3 ) P significantly neutralizes positive potential in the region of the hydrophobic residues , which acts as an `` electrostatic switch '' by reducing the energetic barrier for membrane penetration .
	manualset3
261853	16	424139	15	NULL	NULL	NULL	NULL	observation	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the computational analysis , it is found that ( 1 ) recruitment to membranes is facilitated by non-specific electrostatic interactions that occur between basic residues on the domains and acidic phospholipids in the membrane , ( 2 ) the energetic analysis can quantitatively differentiate among the modes of membrane association proposed by the experimentally determined structures , ( 3 ) FDPB calculations predict energetically feasible models for the membrane-associated states of FYVE domains , ( 4 ) these models are consistent with the observation that conserved hydrophobic residues insert into the membrane interface , and ( 5 ) the calculations provide a molecular model for the hydrophobic partitioning : binding of PI ( 3 ) P significantly neutralizes positive potential in the region of the hydrophobic residues , which acts as an `` electrostatic switch '' by reducing the energetic barrier for membrane penetration .
	manualset3
261855	17	424139	15	NULL	NULL	NULL	NULL	conserved hydrophobic residues	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the computational analysis , it is found that ( 1 ) recruitment to membranes is facilitated by non-specific electrostatic interactions that occur between basic residues on the domains and acidic phospholipids in the membrane , ( 2 ) the energetic analysis can quantitatively differentiate among the modes of membrane association proposed by the experimentally determined structures , ( 3 ) FDPB calculations predict energetically feasible models for the membrane-associated states of FYVE domains , ( 4 ) these models are consistent with the observation that conserved hydrophobic residues insert into the membrane interface , and ( 5 ) the calculations provide a molecular model for the hydrophobic partitioning : binding of PI ( 3 ) P significantly neutralizes positive potential in the region of the hydrophobic residues , which acts as an `` electrostatic switch '' by reducing the energetic barrier for membrane penetration .
	manualset3
261856	18	424139	15	NULL	NULL	NULL	NULL	membrane interface	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the computational analysis , it is found that ( 1 ) recruitment to membranes is facilitated by non-specific electrostatic interactions that occur between basic residues on the domains and acidic phospholipids in the membrane , ( 2 ) the energetic analysis can quantitatively differentiate among the modes of membrane association proposed by the experimentally determined structures , ( 3 ) FDPB calculations predict energetically feasible models for the membrane-associated states of FYVE domains , ( 4 ) these models are consistent with the observation that conserved hydrophobic residues insert into the membrane interface , and ( 5 ) the calculations provide a molecular model for the hydrophobic partitioning : binding of PI ( 3 ) P significantly neutralizes positive potential in the region of the hydrophobic residues , which acts as an `` electrostatic switch '' by reducing the energetic barrier for membrane penetration .
	manualset3
261857	19	424139	15	NULL	NULL	NULL	NULL	calculations	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the computational analysis , it is found that ( 1 ) recruitment to membranes is facilitated by non-specific electrostatic interactions that occur between basic residues on the domains and acidic phospholipids in the membrane , ( 2 ) the energetic analysis can quantitatively differentiate among the modes of membrane association proposed by the experimentally determined structures , ( 3 ) FDPB calculations predict energetically feasible models for the membrane-associated states of FYVE domains , ( 4 ) these models are consistent with the observation that conserved hydrophobic residues insert into the membrane interface , and ( 5 ) the calculations provide a molecular model for the hydrophobic partitioning : binding of PI ( 3 ) P significantly neutralizes positive potential in the region of the hydrophobic residues , which acts as an `` electrostatic switch '' by reducing the energetic barrier for membrane penetration .
	manualset3
261858	20	424139	15	NULL	NULL	NULL	NULL	molecular model	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the computational analysis , it is found that ( 1 ) recruitment to membranes is facilitated by non-specific electrostatic interactions that occur between basic residues on the domains and acidic phospholipids in the membrane , ( 2 ) the energetic analysis can quantitatively differentiate among the modes of membrane association proposed by the experimentally determined structures , ( 3 ) FDPB calculations predict energetically feasible models for the membrane-associated states of FYVE domains , ( 4 ) these models are consistent with the observation that conserved hydrophobic residues insert into the membrane interface , and ( 5 ) the calculations provide a molecular model for the hydrophobic partitioning : binding of PI ( 3 ) P significantly neutralizes positive potential in the region of the hydrophobic residues , which acts as an `` electrostatic switch '' by reducing the energetic barrier for membrane penetration .
	manualset3
261859	21	424139	15	NULL	NULL	NULL	NULL	hydrophobic partitioning	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the computational analysis , it is found that ( 1 ) recruitment to membranes is facilitated by non-specific electrostatic interactions that occur between basic residues on the domains and acidic phospholipids in the membrane , ( 2 ) the energetic analysis can quantitatively differentiate among the modes of membrane association proposed by the experimentally determined structures , ( 3 ) FDPB calculations predict energetically feasible models for the membrane-associated states of FYVE domains , ( 4 ) these models are consistent with the observation that conserved hydrophobic residues insert into the membrane interface , and ( 5 ) the calculations provide a molecular model for the hydrophobic partitioning : binding of PI ( 3 ) P significantly neutralizes positive potential in the region of the hydrophobic residues , which acts as an `` electrostatic switch '' by reducing the energetic barrier for membrane penetration .
	manualset3
261860	22	424139	15	NULL	NULL	NULL	NULL	binding of PI ( 3 ) P	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the computational analysis , it is found that ( 1 ) recruitment to membranes is facilitated by non-specific electrostatic interactions that occur between basic residues on the domains and acidic phospholipids in the membrane , ( 2 ) the energetic analysis can quantitatively differentiate among the modes of membrane association proposed by the experimentally determined structures , ( 3 ) FDPB calculations predict energetically feasible models for the membrane-associated states of FYVE domains , ( 4 ) these models are consistent with the observation that conserved hydrophobic residues insert into the membrane interface , and ( 5 ) the calculations provide a molecular model for the hydrophobic partitioning : binding of PI ( 3 ) P significantly neutralizes positive potential in the region of the hydrophobic residues , which acts as an `` electrostatic switch '' by reducing the energetic barrier for membrane penetration .
	manualset3
261862	23	424139	15	NULL	NULL	NULL	NULL	positive potential	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the computational analysis , it is found that ( 1 ) recruitment to membranes is facilitated by non-specific electrostatic interactions that occur between basic residues on the domains and acidic phospholipids in the membrane , ( 2 ) the energetic analysis can quantitatively differentiate among the modes of membrane association proposed by the experimentally determined structures , ( 3 ) FDPB calculations predict energetically feasible models for the membrane-associated states of FYVE domains , ( 4 ) these models are consistent with the observation that conserved hydrophobic residues insert into the membrane interface , and ( 5 ) the calculations provide a molecular model for the hydrophobic partitioning : binding of PI ( 3 ) P significantly neutralizes positive potential in the region of the hydrophobic residues , which acts as an `` electrostatic switch '' by reducing the energetic barrier for membrane penetration .
	manualset3
261864	24	424139	15	NULL	NULL	NULL	NULL	region	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the computational analysis , it is found that ( 1 ) recruitment to membranes is facilitated by non-specific electrostatic interactions that occur between basic residues on the domains and acidic phospholipids in the membrane , ( 2 ) the energetic analysis can quantitatively differentiate among the modes of membrane association proposed by the experimentally determined structures , ( 3 ) FDPB calculations predict energetically feasible models for the membrane-associated states of FYVE domains , ( 4 ) these models are consistent with the observation that conserved hydrophobic residues insert into the membrane interface , and ( 5 ) the calculations provide a molecular model for the hydrophobic partitioning : binding of PI ( 3 ) P significantly neutralizes positive potential in the region of the hydrophobic residues , which acts as an `` electrostatic switch '' by reducing the energetic barrier for membrane penetration .
	manualset3
261866	25	424139	15	NULL	NULL	NULL	NULL	hydrophobic residues	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the computational analysis , it is found that ( 1 ) recruitment to membranes is facilitated by non-specific electrostatic interactions that occur between basic residues on the domains and acidic phospholipids in the membrane , ( 2 ) the energetic analysis can quantitatively differentiate among the modes of membrane association proposed by the experimentally determined structures , ( 3 ) FDPB calculations predict energetically feasible models for the membrane-associated states of FYVE domains , ( 4 ) these models are consistent with the observation that conserved hydrophobic residues insert into the membrane interface , and ( 5 ) the calculations provide a molecular model for the hydrophobic partitioning : binding of PI ( 3 ) P significantly neutralizes positive potential in the region of the hydrophobic residues , which acts as an `` electrostatic switch '' by reducing the energetic barrier for membrane penetration .
	manualset3
261867	26	424139	15	NULL	NULL	NULL	NULL	electrostatic switch	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the computational analysis , it is found that ( 1 ) recruitment to membranes is facilitated by non-specific electrostatic interactions that occur between basic residues on the domains and acidic phospholipids in the membrane , ( 2 ) the energetic analysis can quantitatively differentiate among the modes of membrane association proposed by the experimentally determined structures , ( 3 ) FDPB calculations predict energetically feasible models for the membrane-associated states of FYVE domains , ( 4 ) these models are consistent with the observation that conserved hydrophobic residues insert into the membrane interface , and ( 5 ) the calculations provide a molecular model for the hydrophobic partitioning : binding of PI ( 3 ) P significantly neutralizes positive potential in the region of the hydrophobic residues , which acts as an `` electrostatic switch '' by reducing the energetic barrier for membrane penetration .
	manualset3
261869	27	424139	15	NULL	NULL	NULL	NULL	energetic barrier	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the computational analysis , it is found that ( 1 ) recruitment to membranes is facilitated by non-specific electrostatic interactions that occur between basic residues on the domains and acidic phospholipids in the membrane , ( 2 ) the energetic analysis can quantitatively differentiate among the modes of membrane association proposed by the experimentally determined structures , ( 3 ) FDPB calculations predict energetically feasible models for the membrane-associated states of FYVE domains , ( 4 ) these models are consistent with the observation that conserved hydrophobic residues insert into the membrane interface , and ( 5 ) the calculations provide a molecular model for the hydrophobic partitioning : binding of PI ( 3 ) P significantly neutralizes positive potential in the region of the hydrophobic residues , which acts as an `` electrostatic switch '' by reducing the energetic barrier for membrane penetration .
	manualset3
261871	28	424139	15	NULL	NULL	NULL	NULL	membrane penetration 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the computational analysis , it is found that ( 1 ) recruitment to membranes is facilitated by non-specific electrostatic interactions that occur between basic residues on the domains and acidic phospholipids in the membrane , ( 2 ) the energetic analysis can quantitatively differentiate among the modes of membrane association proposed by the experimentally determined structures , ( 3 ) FDPB calculations predict energetically feasible models for the membrane-associated states of FYVE domains , ( 4 ) these models are consistent with the observation that conserved hydrophobic residues insert into the membrane interface , and ( 5 ) the calculations provide a molecular model for the hydrophobic partitioning : binding of PI ( 3 ) P significantly neutralizes positive potential in the region of the hydrophobic residues , which acts as an `` electrostatic switch '' by reducing the energetic barrier for membrane penetration .
	manualset3
261873	1	424140	15	NULL	NULL	NULL	NULL	helical parameters	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the measured helical parameters of the L and R lattices and the switching model , the twist and curvature calculated for the ten possible supercoils are in quantitative accord with observed supercoiled forms of flagellar filaments .
	manualset3
261874	2	424140	15	NULL	NULL	NULL	NULL	L lattices	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the measured helical parameters of the L and R lattices and the switching model , the twist and curvature calculated for the ten possible supercoils are in quantitative accord with observed supercoiled forms of flagellar filaments .
	manualset3
261876	3	424140	15	NULL	NULL	NULL	NULL	R lattices 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the measured helical parameters of the L and R lattices and the switching model , the twist and curvature calculated for the ten possible supercoils are in quantitative accord with observed supercoiled forms of flagellar filaments .
	manualset3
261878	4	424140	15	NULL	NULL	NULL	NULL	switching model	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the measured helical parameters of the L and R lattices and the switching model , the twist and curvature calculated for the ten possible supercoils are in quantitative accord with observed supercoiled forms of flagellar filaments .
	manualset3
261879	5	424140	15	NULL	NULL	NULL	NULL	twist	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the measured helical parameters of the L and R lattices and the switching model , the twist and curvature calculated for the ten possible supercoils are in quantitative accord with observed supercoiled forms of flagellar filaments .
	manualset3
261881	6	424140	15	NULL	NULL	NULL	NULL	curvature	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the measured helical parameters of the L and R lattices and the switching model , the twist and curvature calculated for the ten possible supercoils are in quantitative accord with observed supercoiled forms of flagellar filaments .
	manualset3
261882	7	424140	15	NULL	NULL	NULL	NULL	ten	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the measured helical parameters of the L and R lattices and the switching model , the twist and curvature calculated for the ten possible supercoils are in quantitative accord with observed supercoiled forms of flagellar filaments .
	manualset3
261884	8	424140	15	NULL	NULL	NULL	NULL	supercoils	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the measured helical parameters of the L and R lattices and the switching model , the twist and curvature calculated for the ten possible supercoils are in quantitative accord with observed supercoiled forms of flagellar filaments .
	manualset3
261885	9	424140	15	NULL	NULL	NULL	NULL	quantitative accord 	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the measured helical parameters of the L and R lattices and the switching model , the twist and curvature calculated for the ten possible supercoils are in quantitative accord with observed supercoiled forms of flagellar filaments .
	manualset3
261886	10	424140	15	NULL	NULL	NULL	NULL	observed supercoiled forms	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the measured helical parameters of the L and R lattices and the switching model , the twist and curvature calculated for the ten possible supercoils are in quantitative accord with observed supercoiled forms of flagellar filaments .
	manualset3
261887	11	424140	15	NULL	NULL	NULL	NULL	flagellar filaments 	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the measured helical parameters of the L and R lattices and the switching model , the twist and curvature calculated for the ten possible supercoils are in quantitative accord with observed supercoiled forms of flagellar filaments .
	manualset3
262263	1	424141	15	NULL	NULL	NULL	NULL	 mode	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the mode of skeletal remodelling in early ontogeny of all teleosts and in later stages of development of teleosts with acellular bone we suggest a link between acellular bone and the predominance of mononucleated osteoclasts , on the one hand , and cellular bone and multinucleated osteoclasts on the other .
	manualset3
262264	2	424141	15	NULL	NULL	NULL	NULL	skeletal remodelling	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the mode of skeletal remodelling in early ontogeny of all teleosts and in later stages of development of teleosts with acellular bone we suggest a link between acellular bone and the predominance of mononucleated osteoclasts , on the one hand , and cellular bone and multinucleated osteoclasts on the other .
	manualset3
262265	3	424141	15	NULL	NULL	NULL	NULL	early ontogeny 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the mode of skeletal remodelling in early ontogeny of all teleosts and in later stages of development of teleosts with acellular bone we suggest a link between acellular bone and the predominance of mononucleated osteoclasts , on the one hand , and cellular bone and multinucleated osteoclasts on the other .
	manualset3
262266	4	424141	15	NULL	NULL	NULL	NULL	teleosts	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the mode of skeletal remodelling in early ontogeny of all teleosts and in later stages of development of teleosts with acellular bone we suggest a link between acellular bone and the predominance of mononucleated osteoclasts , on the one hand , and cellular bone and multinucleated osteoclasts on the other .
	manualset3
262267	5	424141	15	NULL	NULL	NULL	NULL	later stages of development	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the mode of skeletal remodelling in early ontogeny of all teleosts and in later stages of development of teleosts with acellular bone we suggest a link between acellular bone and the predominance of mononucleated osteoclasts , on the one hand , and cellular bone and multinucleated osteoclasts on the other .
	manualset3
262268	6	424141	15	NULL	NULL	NULL	NULL	teleosts	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the mode of skeletal remodelling in early ontogeny of all teleosts and in later stages of development of teleosts with acellular bone we suggest a link between acellular bone and the predominance of mononucleated osteoclasts , on the one hand , and cellular bone and multinucleated osteoclasts on the other .
	manualset3
262269	7	424141	15	NULL	NULL	NULL	NULL	acellular bone 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the mode of skeletal remodelling in early ontogeny of all teleosts and in later stages of development of teleosts with acellular bone we suggest a link between acellular bone and the predominance of mononucleated osteoclasts , on the one hand , and cellular bone and multinucleated osteoclasts on the other .
	manualset3
262270	8	424141	15	NULL	NULL	NULL	NULL	link	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the mode of skeletal remodelling in early ontogeny of all teleosts and in later stages of development of teleosts with acellular bone we suggest a link between acellular bone and the predominance of mononucleated osteoclasts , on the one hand , and cellular bone and multinucleated osteoclasts on the other .
	manualset3
262271	9	424141	15	NULL	NULL	NULL	NULL	acellular bone	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the mode of skeletal remodelling in early ontogeny of all teleosts and in later stages of development of teleosts with acellular bone we suggest a link between acellular bone and the predominance of mononucleated osteoclasts , on the one hand , and cellular bone and multinucleated osteoclasts on the other .
	manualset3
262272	10	424141	15	NULL	NULL	NULL	NULL	predominance 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the mode of skeletal remodelling in early ontogeny of all teleosts and in later stages of development of teleosts with acellular bone we suggest a link between acellular bone and the predominance of mononucleated osteoclasts , on the one hand , and cellular bone and multinucleated osteoclasts on the other .
	manualset3
262273	11	424141	15	NULL	NULL	NULL	NULL	mononucleated osteoclasts	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the mode of skeletal remodelling in early ontogeny of all teleosts and in later stages of development of teleosts with acellular bone we suggest a link between acellular bone and the predominance of mononucleated osteoclasts , on the one hand , and cellular bone and multinucleated osteoclasts on the other .
	manualset3
262274	12	424141	15	NULL	NULL	NULL	NULL	cellular bone 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the mode of skeletal remodelling in early ontogeny of all teleosts and in later stages of development of teleosts with acellular bone we suggest a link between acellular bone and the predominance of mononucleated osteoclasts , on the one hand , and cellular bone and multinucleated osteoclasts on the other .
	manualset3
262275	13	424141	15	NULL	NULL	NULL	NULL	multinucleated osteoclasts	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the mode of skeletal remodelling in early ontogeny of all teleosts and in later stages of development of teleosts with acellular bone we suggest a link between acellular bone and the predominance of mononucleated osteoclasts , on the one hand , and cellular bone and multinucleated osteoclasts on the other .
	manualset3
262276	1	424142	15	NULL	NULL	NULL	NULL	previous model study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the previous model study , an electroplating industrial effluent was successfully treated with WBAP to minimize the pollution load caused by Ni ( II ) .
	manualset3
262277	2	424142	15	NULL	NULL	NULL	NULL	electroplating industrial effluent	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the previous model study , an electroplating industrial effluent was successfully treated with WBAP to minimize the pollution load caused by Ni ( II ) .
	manualset3
262278	3	424142	15	NULL	NULL	NULL	NULL	WBAP	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the previous model study , an electroplating industrial effluent was successfully treated with WBAP to minimize the pollution load caused by Ni ( II ) .
	manualset3
262279	4	424142	15	NULL	NULL	NULL	NULL	pollution load	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the previous model study , an electroplating industrial effluent was successfully treated with WBAP to minimize the pollution load caused by Ni ( II ) .
	manualset3
262280	5	424142	15	NULL	NULL	NULL	NULL	Ni ( II )	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the previous model study , an electroplating industrial effluent was successfully treated with WBAP to minimize the pollution load caused by Ni ( II ) .
	manualset3
262281	1	424143	15	NULL	NULL	NULL	NULL	proteomic literature 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the previously published proteomic and genomic literature on S. oneidensis , this reduction in power output is most likely due to the differential expression of proteins by these bacteria when grown under oxygen-rich or anoxic conditions .
	manualset3
262282	2	424143	15	NULL	NULL	NULL	NULL	genomic literature	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the previously published proteomic and genomic literature on S. oneidensis , this reduction in power output is most likely due to the differential expression of proteins by these bacteria when grown under oxygen-rich or anoxic conditions .
	manualset3
262283	3	424143	15	NULL	NULL	NULL	NULL	S. oneidensis	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the previously published proteomic and genomic literature on S. oneidensis , this reduction in power output is most likely due to the differential expression of proteins by these bacteria when grown under oxygen-rich or anoxic conditions .
	manualset3
262284	4	424143	15	NULL	NULL	NULL	NULL	reduction in power output	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the previously published proteomic and genomic literature on S. oneidensis , this reduction in power output is most likely due to the differential expression of proteins by these bacteria when grown under oxygen-rich or anoxic conditions .
	manualset3
262285	5	424143	15	NULL	NULL	NULL	NULL	differential expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the previously published proteomic and genomic literature on S. oneidensis , this reduction in power output is most likely due to the differential expression of proteins by these bacteria when grown under oxygen-rich or anoxic conditions .
	manualset3
262286	6	424143	15	NULL	NULL	NULL	NULL	proteins 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the previously published proteomic and genomic literature on S. oneidensis , this reduction in power output is most likely due to the differential expression of proteins by these bacteria when grown under oxygen-rich or anoxic conditions .
	manualset3
262287	7	424143	15	NULL	NULL	NULL	NULL	 bacteria	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the previously published proteomic and genomic literature on S. oneidensis , this reduction in power output is most likely due to the differential expression of proteins by these bacteria when grown under oxygen-rich or anoxic conditions .
	manualset3
262288	8	424143	15	NULL	NULL	NULL	NULL	oxygen-rich conditions	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the previously published proteomic and genomic literature on S. oneidensis , this reduction in power output is most likely due to the differential expression of proteins by these bacteria when grown under oxygen-rich or anoxic conditions .
	manualset3
262289	9	424143	15	NULL	NULL	NULL	NULL	anoxic conditions	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the previously published proteomic and genomic literature on S. oneidensis , this reduction in power output is most likely due to the differential expression of proteins by these bacteria when grown under oxygen-rich or anoxic conditions .
	manualset3
262290	1	424144	15	NULL	NULL	NULL	NULL	position	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the relative position of exposed or hidden regions of the individual components in the complex derived from their tryptic susceptibilities , an assembly model is proposed for the arrangement of individual subunits in the botulinum L-TC .
	manualset3
262291	2	424144	15	NULL	NULL	NULL	NULL	exposed regions	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the relative position of exposed or hidden regions of the individual components in the complex derived from their tryptic susceptibilities , an assembly model is proposed for the arrangement of individual subunits in the botulinum L-TC .
	manualset3
262292	3	424144	15	NULL	NULL	NULL	NULL	hidden regions	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the relative position of exposed or hidden regions of the individual components in the complex derived from their tryptic susceptibilities , an assembly model is proposed for the arrangement of individual subunits in the botulinum L-TC .
	manualset3
262293	4	424144	15	NULL	NULL	NULL	NULL	individual components	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the relative position of exposed or hidden regions of the individual components in the complex derived from their tryptic susceptibilities , an assembly model is proposed for the arrangement of individual subunits in the botulinum L-TC .
	manualset3
262294	5	424144	15	NULL	NULL	NULL	NULL	complex	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the relative position of exposed or hidden regions of the individual components in the complex derived from their tryptic susceptibilities , an assembly model is proposed for the arrangement of individual subunits in the botulinum L-TC .
	manualset3
262295	6	424144	15	NULL	NULL	NULL	NULL	tryptic susceptibilities	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the relative position of exposed or hidden regions of the individual components in the complex derived from their tryptic susceptibilities , an assembly model is proposed for the arrangement of individual subunits in the botulinum L-TC .
	manualset3
262296	7	424144	15	NULL	NULL	NULL	NULL	assembly model	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the relative position of exposed or hidden regions of the individual components in the complex derived from their tryptic susceptibilities , an assembly model is proposed for the arrangement of individual subunits in the botulinum L-TC .
	manualset3
262297	8	424144	15	NULL	NULL	NULL	NULL	arrangement	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the relative position of exposed or hidden regions of the individual components in the complex derived from their tryptic susceptibilities , an assembly model is proposed for the arrangement of individual subunits in the botulinum L-TC .
	manualset3
262298	9	424144	15	NULL	NULL	NULL	NULL	individual subunits	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the relative position of exposed or hidden regions of the individual components in the complex derived from their tryptic susceptibilities , an assembly model is proposed for the arrangement of individual subunits in the botulinum L-TC .
	manualset3
262299	10	424144	15	NULL	NULL	NULL	NULL	botulinum L-TC	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the relative position of exposed or hidden regions of the individual components in the complex derived from their tryptic susceptibilities , an assembly model is proposed for the arrangement of individual subunits in the botulinum L-TC .
	manualset3
262300	1	424145	15	NULL	NULL	NULL	NULL	Experimental lung graft	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental lung graft using the Nakayama fastener ) .
	manualset3
262301	2	424145	15	NULL	NULL	NULL	NULL	Nakayama fastener	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental lung graft using the Nakayama fastener ) .
	manualset3
262302	1	424146	15	NULL	NULL	NULL	NULL	energy production rate	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the same energy production rate , the land application of SNO FGD material from Plant S released higher amounts of Hg and B into ambient air and/or grass than the amounts released when AFO-gypsum from Plant A was used .
	manualset3
262303	2	424146	15	NULL	NULL	NULL	NULL	land application 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the same energy production rate , the land application of SNO FGD material from Plant S released higher amounts of Hg and B into ambient air and/or grass than the amounts released when AFO-gypsum from Plant A was used .
	manualset3
262304	3	424146	15	NULL	NULL	NULL	NULL	SNO FGD material	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the same energy production rate , the land application of SNO FGD material from Plant S released higher amounts of Hg and B into ambient air and/or grass than the amounts released when AFO-gypsum from Plant A was used .
	manualset3
262305	4	424146	15	NULL	NULL	NULL	NULL	Plant S	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the same energy production rate , the land application of SNO FGD material from Plant S released higher amounts of Hg and B into ambient air and/or grass than the amounts released when AFO-gypsum from Plant A was used .
	manualset3
262306	5	424146	15	NULL	NULL	NULL	NULL	amounts	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the same energy production rate , the land application of SNO FGD material from Plant S released higher amounts of Hg and B into ambient air and/or grass than the amounts released when AFO-gypsum from Plant A was used .
	manualset3
262307	6	424146	15	NULL	NULL	NULL	NULL	Hg	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the same energy production rate , the land application of SNO FGD material from Plant S released higher amounts of Hg and B into ambient air and/or grass than the amounts released when AFO-gypsum from Plant A was used .
	manualset3
262308	7	424146	15	NULL	NULL	NULL	NULL	B	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the same energy production rate , the land application of SNO FGD material from Plant S released higher amounts of Hg and B into ambient air and/or grass than the amounts released when AFO-gypsum from Plant A was used .
	manualset3
262309	8	424146	15	NULL	NULL	NULL	NULL	ambient air	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the same energy production rate , the land application of SNO FGD material from Plant S released higher amounts of Hg and B into ambient air and/or grass than the amounts released when AFO-gypsum from Plant A was used .
	manualset3
262310	9	424146	15	NULL	NULL	NULL	NULL	grass	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the same energy production rate , the land application of SNO FGD material from Plant S released higher amounts of Hg and B into ambient air and/or grass than the amounts released when AFO-gypsum from Plant A was used .
	manualset3
262311	10	424146	15	NULL	NULL	NULL	NULL	amounts	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the same energy production rate , the land application of SNO FGD material from Plant S released higher amounts of Hg and B into ambient air and/or grass than the amounts released when AFO-gypsum from Plant A was used .
	manualset3
262312	11	424146	15	NULL	NULL	NULL	NULL	AFO-gypsum	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the same energy production rate , the land application of SNO FGD material from Plant S released higher amounts of Hg and B into ambient air and/or grass than the amounts released when AFO-gypsum from Plant A was used .
	manualset3
262313	12	424146	15	NULL	NULL	NULL	NULL	Plant A	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the same energy production rate , the land application of SNO FGD material from Plant S released higher amounts of Hg and B into ambient air and/or grass than the amounts released when AFO-gypsum from Plant A was used .
	manualset3
262314	1	424147	15	NULL	NULL	NULL	NULL	subchronic study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the subchronic study , the no observed-adverse-effect level ( NOAEL ) for mushroom - glucan was determined as 2000 mg/kgbw/day , the highest dose tested .
	manualset3
262315	2	424147	15	NULL	NULL	NULL	NULL	no observed-adverse-effect level ( NOAEL )	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the subchronic study , the no observed-adverse-effect level ( NOAEL ) for mushroom - glucan was determined as 2000 mg/kgbw/day , the highest dose tested .
	manualset3
262316	3	424147	15	NULL	NULL	NULL	NULL	mushroom - glucan	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the subchronic study , the no observed-adverse-effect level ( NOAEL ) for mushroom - glucan was determined as 2000 mg/kgbw/day , the highest dose tested .
	manualset3
262317	4	424147	15	NULL	NULL	NULL	NULL	2000 mg/kgbw/day	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the subchronic study , the no observed-adverse-effect level ( NOAEL ) for mushroom - glucan was determined as 2000 mg/kgbw/day , the highest dose tested .
	manualset3
262318	5	424147	15	NULL	NULL	NULL	NULL	dose	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the subchronic study , the no observed-adverse-effect level ( NOAEL ) for mushroom - glucan was determined as 2000 mg/kgbw/day , the highest dose tested .
	manualset3
262319	1	424148	15	NULL	NULL	NULL	NULL	survey	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the survey of the fishes in low salinity intertidal area of the Yangtze estuary from spring ( May ) 2006 to winter ( February ) 2007 , the seasonal and semi-lunar changes of fish species and abundances were analyzed .
	manualset3
262320	2	424148	15	NULL	NULL	NULL	NULL	fishes	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the survey of the fishes in low salinity intertidal area of the Yangtze estuary from spring ( May ) 2006 to winter ( February ) 2007 , the seasonal and semi-lunar changes of fish species and abundances were analyzed .
	manualset3
262321	3	424148	15	NULL	NULL	NULL	NULL	low salinity intertidal area 	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the survey of the fishes in low salinity intertidal area of the Yangtze estuary from spring ( May ) 2006 to winter ( February ) 2007 , the seasonal and semi-lunar changes of fish species and abundances were analyzed .
	manualset3
262322	4	424148	15	NULL	NULL	NULL	NULL	Yangtze estuary	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the survey of the fishes in low salinity intertidal area of the Yangtze estuary from spring ( May ) 2006 to winter ( February ) 2007 , the seasonal and semi-lunar changes of fish species and abundances were analyzed .
	manualset3
262323	5	424148	15	NULL	NULL	NULL	NULL	spring ( May ) 2006 to winter ( February ) 2007 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the survey of the fishes in low salinity intertidal area of the Yangtze estuary from spring ( May ) 2006 to winter ( February ) 2007 , the seasonal and semi-lunar changes of fish species and abundances were analyzed .
	manualset3
262324	6	424148	15	NULL	NULL	NULL	NULL	seasonal changes 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the survey of the fishes in low salinity intertidal area of the Yangtze estuary from spring ( May ) 2006 to winter ( February ) 2007 , the seasonal and semi-lunar changes of fish species and abundances were analyzed .
	manualset3
262325	7	424148	15	NULL	NULL	NULL	NULL	semi-lunar changes	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the survey of the fishes in low salinity intertidal area of the Yangtze estuary from spring ( May ) 2006 to winter ( February ) 2007 , the seasonal and semi-lunar changes of fish species and abundances were analyzed .
	manualset3
262326	8	424148	15	NULL	NULL	NULL	NULL	fish species	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the survey of the fishes in low salinity intertidal area of the Yangtze estuary from spring ( May ) 2006 to winter ( February ) 2007 , the seasonal and semi-lunar changes of fish species and abundances were analyzed .
	manualset3
262327	9	424148	15	NULL	NULL	NULL	NULL	abundances	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on the survey of the fishes in low salinity intertidal area of the Yangtze estuary from spring ( May ) 2006 to winter ( February ) 2007 , the seasonal and semi-lunar changes of fish species and abundances were analyzed .
	manualset3
262328	1	424149	15	NULL	NULL	NULL	NULL	amino acid sequence	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on their amino acid sequence identity and enzyme activity assay , the gene products were identified as dihydropyrimidine dehydrogenase ( PydA ) , dihydropyrimidinase ( PydB ) , and beta-alanine synthase ( PydC ) .
	manualset3
262329	2	424149	15	NULL	NULL	NULL	NULL	enzyme activity assay	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on their amino acid sequence identity and enzyme activity assay , the gene products were identified as dihydropyrimidine dehydrogenase ( PydA ) , dihydropyrimidinase ( PydB ) , and beta-alanine synthase ( PydC ) .
	manualset3
262330	3	424149	15	NULL	NULL	NULL	NULL	gene products	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on their amino acid sequence identity and enzyme activity assay , the gene products were identified as dihydropyrimidine dehydrogenase ( PydA ) , dihydropyrimidinase ( PydB ) , and beta-alanine synthase ( PydC ) .
	manualset3
262331	4	424149	15	NULL	NULL	NULL	NULL	dihydropyrimidine dehydrogenase ( PydA )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on their amino acid sequence identity and enzyme activity assay , the gene products were identified as dihydropyrimidine dehydrogenase ( PydA ) , dihydropyrimidinase ( PydB ) , and beta-alanine synthase ( PydC ) .
	manualset3
262332	5	424149	15	NULL	NULL	NULL	NULL	dihydropyrimidinase ( PydB )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on their amino acid sequence identity and enzyme activity assay , the gene products were identified as dihydropyrimidine dehydrogenase ( PydA ) , dihydropyrimidinase ( PydB ) , and beta-alanine synthase ( PydC ) .
	manualset3
262333	6	424149	15	NULL	NULL	NULL	NULL	beta-alanine synthase ( PydC )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on their amino acid sequence identity and enzyme activity assay , the gene products were identified as dihydropyrimidine dehydrogenase ( PydA ) , dihydropyrimidinase ( PydB ) , and beta-alanine synthase ( PydC ) .
	manualset3
262334	1	424150	15	NULL	NULL	NULL	NULL	case reports	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these case reports and the medical literature on pneumocephalus , we review the causes and treatment of this rare condition .
	manualset3
262335	2	424150	15	NULL	NULL	NULL	NULL	medical literature 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these case reports and the medical literature on pneumocephalus , we review the causes and treatment of this rare condition .
	manualset3
262336	3	424150	15	NULL	NULL	NULL	NULL	pneumocephalus	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these case reports and the medical literature on pneumocephalus , we review the causes and treatment of this rare condition .
	manualset3
262337	4	424150	15	NULL	NULL	NULL	NULL	causes	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these case reports and the medical literature on pneumocephalus , we review the causes and treatment of this rare condition .
	manualset3
262338	5	424150	15	NULL	NULL	NULL	NULL	treatment 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these case reports and the medical literature on pneumocephalus , we review the causes and treatment of this rare condition .
	manualset3
262339	6	424150	15	NULL	NULL	NULL	NULL	rare condition	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these case reports and the medical literature on pneumocephalus , we review the causes and treatment of this rare condition .
	manualset3
262340	1	424151	15	NULL	NULL	NULL	NULL	findings 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these findings , Rg5 can ameliorate lung inflammation possibly by inhibiting the binding of LPS to toll-like receptor ( TLR ) -4 on macrophages .
	manualset3
262341	2	424151	15	NULL	NULL	NULL	NULL	Rg5	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these findings , Rg5 can ameliorate lung inflammation possibly by inhibiting the binding of LPS to toll-like receptor ( TLR ) -4 on macrophages .
	manualset3
262342	3	424151	15	NULL	NULL	NULL	NULL	lung inflammation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these findings , Rg5 can ameliorate lung inflammation possibly by inhibiting the binding of LPS to toll-like receptor ( TLR ) -4 on macrophages .
	manualset3
262343	4	424151	15	NULL	NULL	NULL	NULL	binding of LPS	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these findings , Rg5 can ameliorate lung inflammation possibly by inhibiting the binding of LPS to toll-like receptor ( TLR ) -4 on macrophages .
	manualset3
262344	5	424151	15	NULL	NULL	NULL	NULL	toll-like receptor ( TLR ) -4 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these findings , Rg5 can ameliorate lung inflammation possibly by inhibiting the binding of LPS to toll-like receptor ( TLR ) -4 on macrophages .
	manualset3
262345	6	424151	15	NULL	NULL	NULL	NULL	macrophages	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these findings , Rg5 can ameliorate lung inflammation possibly by inhibiting the binding of LPS to toll-like receptor ( TLR ) -4 on macrophages .
	manualset3
262346	1	424152	15	NULL	NULL	NULL	NULL	first congener-specific dioxin analyses	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these first congener-specific dioxin analyses of U.S. food , U.S. average daily intake of `` International '' dioxin toxic equivalents for an adult weighing 65 kilograms ( kg ) was estimated to be between 18 to 192 picograms TEq or 0.3 to 3.0 picograms per kilogram of body weight .
	manualset3
262347	2	424152	15	NULL	NULL	NULL	NULL	U.S. food	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these first congener-specific dioxin analyses of U.S. food , U.S. average daily intake of `` International '' dioxin toxic equivalents for an adult weighing 65 kilograms ( kg ) was estimated to be between 18 to 192 picograms TEq or 0.3 to 3.0 picograms per kilogram of body weight .
	manualset3
262348	3	424152	15	NULL	NULL	NULL	NULL	U.S. average daily intake	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these first congener-specific dioxin analyses of U.S. food , U.S. average daily intake of `` International '' dioxin toxic equivalents for an adult weighing 65 kilograms ( kg ) was estimated to be between 18 to 192 picograms TEq or 0.3 to 3.0 picograms per kilogram of body weight .
	manualset3
262349	4	424152	15	NULL	NULL	NULL	NULL	`` International '' dioxin toxic equivalents 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these first congener-specific dioxin analyses of U.S. food , U.S. average daily intake of `` International '' dioxin toxic equivalents for an adult weighing 65 kilograms ( kg ) was estimated to be between 18 to 192 picograms TEq or 0.3 to 3.0 picograms per kilogram of body weight .
	manualset3
262350	5	424152	15	NULL	NULL	NULL	NULL	adult 	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these first congener-specific dioxin analyses of U.S. food , U.S. average daily intake of `` International '' dioxin toxic equivalents for an adult weighing 65 kilograms ( kg ) was estimated to be between 18 to 192 picograms TEq or 0.3 to 3.0 picograms per kilogram of body weight .
	manualset3
262351	6	424152	15	NULL	NULL	NULL	NULL	65 kilograms ( kg )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these first congener-specific dioxin analyses of U.S. food , U.S. average daily intake of `` International '' dioxin toxic equivalents for an adult weighing 65 kilograms ( kg ) was estimated to be between 18 to 192 picograms TEq or 0.3 to 3.0 picograms per kilogram of body weight .
	manualset3
262352	7	424152	15	NULL	NULL	NULL	NULL	18 picograms TEq	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these first congener-specific dioxin analyses of U.S. food , U.S. average daily intake of `` International '' dioxin toxic equivalents for an adult weighing 65 kilograms ( kg ) was estimated to be between 18 to 192 picograms TEq or 0.3 to 3.0 picograms per kilogram of body weight .
	manualset3
262353	8	424152	15	NULL	NULL	NULL	NULL	192 picograms TEq 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these first congener-specific dioxin analyses of U.S. food , U.S. average daily intake of `` International '' dioxin toxic equivalents for an adult weighing 65 kilograms ( kg ) was estimated to be between 18 to 192 picograms TEq or 0.3 to 3.0 picograms per kilogram of body weight .
	manualset3
262354	9	424152	15	NULL	NULL	NULL	NULL	0.3 picograms per kilogram of body weight	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these first congener-specific dioxin analyses of U.S. food , U.S. average daily intake of `` International '' dioxin toxic equivalents for an adult weighing 65 kilograms ( kg ) was estimated to be between 18 to 192 picograms TEq or 0.3 to 3.0 picograms per kilogram of body weight .
	manualset3
262355	10	424152	15	NULL	NULL	NULL	NULL	3.0 picograms per kilogram of body weight	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these first congener-specific dioxin analyses of U.S. food , U.S. average daily intake of `` International '' dioxin toxic equivalents for an adult weighing 65 kilograms ( kg ) was estimated to be between 18 to 192 picograms TEq or 0.3 to 3.0 picograms per kilogram of body weight .
	manualset3
262356	1	424153	15	NULL	NULL	NULL	NULL	formulas	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these formulas , the structural parameters of ligand octahedra of Co2 + in Rb2MgF4 crystal are obtained by fitting the calculated g ( parallel ) and g ( perpendicular ) to the observed values .
	manualset3
262357	2	424153	15	NULL	NULL	NULL	NULL	structural parameters	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these formulas , the structural parameters of ligand octahedra of Co2 + in Rb2MgF4 crystal are obtained by fitting the calculated g ( parallel ) and g ( perpendicular ) to the observed values .
	manualset3
262358	3	424153	15	NULL	NULL	NULL	NULL	ligand octahedra	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these formulas , the structural parameters of ligand octahedra of Co2 + in Rb2MgF4 crystal are obtained by fitting the calculated g ( parallel ) and g ( perpendicular ) to the observed values .
	manualset3
262359	4	424153	15	NULL	NULL	NULL	NULL	Co2 +	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these formulas , the structural parameters of ligand octahedra of Co2 + in Rb2MgF4 crystal are obtained by fitting the calculated g ( parallel ) and g ( perpendicular ) to the observed values .
	manualset3
262360	5	424153	15	NULL	NULL	NULL	NULL	Rb2MgF4 crystal	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these formulas , the structural parameters of ligand octahedra of Co2 + in Rb2MgF4 crystal are obtained by fitting the calculated g ( parallel ) and g ( perpendicular ) to the observed values .
	manualset3
262361	6	424153	15	NULL	NULL	NULL	NULL	g ( parallel )	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these formulas , the structural parameters of ligand octahedra of Co2 + in Rb2MgF4 crystal are obtained by fitting the calculated g ( parallel ) and g ( perpendicular ) to the observed values .
	manualset3
262362	7	424153	15	NULL	NULL	NULL	NULL	g ( perpendicular ) 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these formulas , the structural parameters of ligand octahedra of Co2 + in Rb2MgF4 crystal are obtained by fitting the calculated g ( parallel ) and g ( perpendicular ) to the observed values .
	manualset3
262363	8	424153	15	NULL	NULL	NULL	NULL	values	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these formulas , the structural parameters of ligand octahedra of Co2 + in Rb2MgF4 crystal are obtained by fitting the calculated g ( parallel ) and g ( perpendicular ) to the observed values .
	manualset3
262364	1	424154	15	NULL	NULL	NULL	NULL	Experimental pathogenicity 	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental pathogenicity in mice of poliovirus 2 strains ) .
	manualset3
262365	2	424154	15	NULL	NULL	NULL	NULL	mice 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental pathogenicity in mice of poliovirus 2 strains ) .
	manualset3
262366	3	424154	15	NULL	NULL	NULL	NULL	poliovirus 2 strains	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental pathogenicity in mice of poliovirus 2 strains ) .
	manualset3
262367	1	424155	15	NULL	NULL	NULL	NULL	observations 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these observations , we hypothesized that Rck may also possess this ability .
	manualset3
262368	2	424155	15	NULL	NULL	NULL	NULL	Rck	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these observations , we hypothesized that Rck may also possess this ability .
	manualset3
262369	3	424155	15	NULL	NULL	NULL	NULL	ability	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these observations , we hypothesized that Rck may also possess this ability .
	manualset3
262370	1	424156	15	NULL	NULL	NULL	NULL	results	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , PDT was performed on HCC at 3 h after 500 mg x kg ( -1 ) ALA administration before laser irradiation of 30 J per tumor .
	manualset3
262371	2	424156	15	NULL	NULL	NULL	NULL	PDT	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , PDT was performed on HCC at 3 h after 500 mg x kg ( -1 ) ALA administration before laser irradiation of 30 J per tumor .
	manualset3
262449	3	424156	15	NULL	NULL	NULL	NULL	HCC	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , PDT was performed on HCC at 3 h after 500 mg x kg ( -1 ) ALA administration before laser irradiation of 30 J per tumor .
	manualset3
262452	4	424156	15	NULL	NULL	NULL	NULL	3 h	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , PDT was performed on HCC at 3 h after 500 mg x kg ( -1 ) ALA administration before laser irradiation of 30 J per tumor .
	manualset3
262454	5	424156	15	NULL	NULL	NULL	NULL	500 mg x kg ( -1 ) 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , PDT was performed on HCC at 3 h after 500 mg x kg ( -1 ) ALA administration before laser irradiation of 30 J per tumor .
	manualset3
262458	6	424156	15	NULL	NULL	NULL	NULL	ALA administration	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , PDT was performed on HCC at 3 h after 500 mg x kg ( -1 ) ALA administration before laser irradiation of 30 J per tumor .
	manualset3
262462	7	424156	15	NULL	NULL	NULL	NULL	laser irradiation 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , PDT was performed on HCC at 3 h after 500 mg x kg ( -1 ) ALA administration before laser irradiation of 30 J per tumor .
	manualset3
262465	8	424156	15	NULL	NULL	NULL	NULL	30 J 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , PDT was performed on HCC at 3 h after 500 mg x kg ( -1 ) ALA administration before laser irradiation of 30 J per tumor .
	manualset3
262466	9	424156	15	NULL	NULL	NULL	NULL	tumor 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , PDT was performed on HCC at 3 h after 500 mg x kg ( -1 ) ALA administration before laser irradiation of 30 J per tumor .
	manualset3
262471	1	424157	15	NULL	NULL	NULL	NULL	results 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , T-CAM can be applied where enhancement of cell adhesion , migration and proliferation are desired , and it could be developed into novel wound healing drug .
	manualset3
262472	2	424157	15	NULL	NULL	NULL	NULL	T-CAM	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , T-CAM can be applied where enhancement of cell adhesion , migration and proliferation are desired , and it could be developed into novel wound healing drug .
	manualset3
262473	3	424157	15	NULL	NULL	NULL	NULL	enhancement of cell adhesion	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , T-CAM can be applied where enhancement of cell adhesion , migration and proliferation are desired , and it could be developed into novel wound healing drug .
	manualset3
262475	4	424157	15	NULL	NULL	NULL	NULL	migration	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , T-CAM can be applied where enhancement of cell adhesion , migration and proliferation are desired , and it could be developed into novel wound healing drug .
	manualset3
262477	5	424157	15	NULL	NULL	NULL	NULL	proliferation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , T-CAM can be applied where enhancement of cell adhesion , migration and proliferation are desired , and it could be developed into novel wound healing drug .
	manualset3
262479	6	424157	15	NULL	NULL	NULL	NULL	wound healing drug	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , T-CAM can be applied where enhancement of cell adhesion , migration and proliferation are desired , and it could be developed into novel wound healing drug .
	manualset3
262480	1	424158	15	NULL	NULL	NULL	NULL	results	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , Tth was selected as the most suitable enzyme for the assay .
	manualset3
262481	2	424158	15	NULL	NULL	NULL	NULL	Tth	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , Tth was selected as the most suitable enzyme for the assay .
	manualset3
262482	3	424158	15	NULL	NULL	NULL	NULL	enzyme	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , Tth was selected as the most suitable enzyme for the assay .
	manualset3
262483	4	424158	15	NULL	NULL	NULL	NULL	assay	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , Tth was selected as the most suitable enzyme for the assay .
	manualset3
262484	1	424159	15	NULL	NULL	NULL	NULL	results	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , a con-ceivable pathway for the formation of 2 ' - deoxyoxanosine from 2 ' - deoxyguanosine by HNO ( 2 ) is proposed .
	manualset3
262485	2	424159	15	NULL	NULL	NULL	NULL	con-ceivable pathway	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , a con-ceivable pathway for the formation of 2 ' - deoxyoxanosine from 2 ' - deoxyguanosine by HNO ( 2 ) is proposed .
	manualset3
262486	3	424159	15	NULL	NULL	NULL	NULL	formation of 2 ' - deoxyoxanosine	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , a con-ceivable pathway for the formation of 2 ' - deoxyoxanosine from 2 ' - deoxyguanosine by HNO ( 2 ) is proposed .
	manualset3
262487	4	424159	15	NULL	NULL	NULL	NULL	2 ' - deoxyguanosine	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , a con-ceivable pathway for the formation of 2 ' - deoxyoxanosine from 2 ' - deoxyguanosine by HNO ( 2 ) is proposed .
	manualset3
262488	5	424159	15	NULL	NULL	NULL	NULL	HNO ( 2 ) 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , a con-ceivable pathway for the formation of 2 ' - deoxyoxanosine from 2 ' - deoxyguanosine by HNO ( 2 ) is proposed .
	manualset3
262489	1	424160	15	NULL	NULL	NULL	NULL	results	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , an additional booster , still a controversial issue , does not appear to be required in order to prevent infection with hepatitis B virus and thus permit the eventual eradication of chronic carriage and its fatal sequelae in Thailand .
	manualset3
262492	2	424160	15	NULL	NULL	NULL	NULL	booster	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , an additional booster , still a controversial issue , does not appear to be required in order to prevent infection with hepatitis B virus and thus permit the eventual eradication of chronic carriage and its fatal sequelae in Thailand .
	manualset3
262494	3	424160	15	NULL	NULL	NULL	NULL	issue	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , an additional booster , still a controversial issue , does not appear to be required in order to prevent infection with hepatitis B virus and thus permit the eventual eradication of chronic carriage and its fatal sequelae in Thailand .
	manualset3
262498	4	424160	15	NULL	NULL	NULL	NULL	infection 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , an additional booster , still a controversial issue , does not appear to be required in order to prevent infection with hepatitis B virus and thus permit the eventual eradication of chronic carriage and its fatal sequelae in Thailand .
	manualset3
262500	5	424160	15	NULL	NULL	NULL	NULL	hepatitis B virus	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , an additional booster , still a controversial issue , does not appear to be required in order to prevent infection with hepatitis B virus and thus permit the eventual eradication of chronic carriage and its fatal sequelae in Thailand .
	manualset3
262503	6	424160	15	NULL	NULL	NULL	NULL	eradication of chronic carriage	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , an additional booster , still a controversial issue , does not appear to be required in order to prevent infection with hepatitis B virus and thus permit the eventual eradication of chronic carriage and its fatal sequelae in Thailand .
	manualset3
262506	7	424160	15	NULL	NULL	NULL	NULL	fatal sequelae	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , an additional booster , still a controversial issue , does not appear to be required in order to prevent infection with hepatitis B virus and thus permit the eventual eradication of chronic carriage and its fatal sequelae in Thailand .
	manualset3
262510	8	424160	15	NULL	NULL	NULL	NULL	Thailand	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , an additional booster , still a controversial issue , does not appear to be required in order to prevent infection with hepatitis B virus and thus permit the eventual eradication of chronic carriage and its fatal sequelae in Thailand .
	manualset3
262512	1	424161	15	NULL	NULL	NULL	NULL	results	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , we propose that decreased cell and body size of the small mutants in the DBL-1 / TGFbeta pathway is mainly due to decreased levels of protein expression , and that increase in fluid content is a major reason for the increase in cell and body size in egl-4 mutants .
	manualset3
262519	2	424161	15	NULL	NULL	NULL	NULL	cell size	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , we propose that decreased cell and body size of the small mutants in the DBL-1 / TGFbeta pathway is mainly due to decreased levels of protein expression , and that increase in fluid content is a major reason for the increase in cell and body size in egl-4 mutants .
	manualset3
262521	3	424161	15	NULL	NULL	NULL	NULL	body size	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , we propose that decreased cell and body size of the small mutants in the DBL-1 / TGFbeta pathway is mainly due to decreased levels of protein expression , and that increase in fluid content is a major reason for the increase in cell and body size in egl-4 mutants .
	manualset3
262524	4	424161	15	NULL	NULL	NULL	NULL	small mutants	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , we propose that decreased cell and body size of the small mutants in the DBL-1 / TGFbeta pathway is mainly due to decreased levels of protein expression , and that increase in fluid content is a major reason for the increase in cell and body size in egl-4 mutants .
	manualset3
262525	5	424161	15	NULL	NULL	NULL	NULL	DBL-1 / TGFbeta pathway	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , we propose that decreased cell and body size of the small mutants in the DBL-1 / TGFbeta pathway is mainly due to decreased levels of protein expression , and that increase in fluid content is a major reason for the increase in cell and body size in egl-4 mutants .
	manualset3
262526	6	424161	15	NULL	NULL	NULL	NULL	levels	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , we propose that decreased cell and body size of the small mutants in the DBL-1 / TGFbeta pathway is mainly due to decreased levels of protein expression , and that increase in fluid content is a major reason for the increase in cell and body size in egl-4 mutants .
	manualset3
262527	7	424161	15	NULL	NULL	NULL	NULL	protein expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , we propose that decreased cell and body size of the small mutants in the DBL-1 / TGFbeta pathway is mainly due to decreased levels of protein expression , and that increase in fluid content is a major reason for the increase in cell and body size in egl-4 mutants .
	manualset3
262530	8	424161	15	NULL	NULL	NULL	NULL	increase	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , we propose that decreased cell and body size of the small mutants in the DBL-1 / TGFbeta pathway is mainly due to decreased levels of protein expression , and that increase in fluid content is a major reason for the increase in cell and body size in egl-4 mutants .
	manualset3
262531	9	424161	15	NULL	NULL	NULL	NULL	fluid content 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , we propose that decreased cell and body size of the small mutants in the DBL-1 / TGFbeta pathway is mainly due to decreased levels of protein expression , and that increase in fluid content is a major reason for the increase in cell and body size in egl-4 mutants .
	manualset3
262560	10	424161	15	NULL	NULL	NULL	NULL	reason	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , we propose that decreased cell and body size of the small mutants in the DBL-1 / TGFbeta pathway is mainly due to decreased levels of protein expression , and that increase in fluid content is a major reason for the increase in cell and body size in egl-4 mutants .
	manualset3
262561	11	424161	15	NULL	NULL	NULL	NULL	 increase 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , we propose that decreased cell and body size of the small mutants in the DBL-1 / TGFbeta pathway is mainly due to decreased levels of protein expression , and that increase in fluid content is a major reason for the increase in cell and body size in egl-4 mutants .
	manualset3
262562	12	424161	15	NULL	NULL	NULL	NULL	cell size	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , we propose that decreased cell and body size of the small mutants in the DBL-1 / TGFbeta pathway is mainly due to decreased levels of protein expression , and that increase in fluid content is a major reason for the increase in cell and body size in egl-4 mutants .
	manualset3
262563	13	424161	15	NULL	NULL	NULL	NULL	body size	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , we propose that decreased cell and body size of the small mutants in the DBL-1 / TGFbeta pathway is mainly due to decreased levels of protein expression , and that increase in fluid content is a major reason for the increase in cell and body size in egl-4 mutants .
	manualset3
262564	14	424161	15	NULL	NULL	NULL	NULL	egl-4 mutants	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results , we propose that decreased cell and body size of the small mutants in the DBL-1 / TGFbeta pathway is mainly due to decreased levels of protein expression , and that increase in fluid content is a major reason for the increase in cell and body size in egl-4 mutants .
	manualset3
262565	1	424162	15	NULL	NULL	NULL	NULL	results 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results we conclude that Fc gamma RII mediate antibody-dependent enhancement of dengue virus infection in addition to Fc gamma RI .
	manualset3
262566	2	424162	15	NULL	NULL	NULL	NULL	Fc gamma RII	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results we conclude that Fc gamma RII mediate antibody-dependent enhancement of dengue virus infection in addition to Fc gamma RI .
	manualset3
262567	3	424162	15	NULL	NULL	NULL	NULL	antibody-dependent enhancement	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results we conclude that Fc gamma RII mediate antibody-dependent enhancement of dengue virus infection in addition to Fc gamma RI .
	manualset3
262568	4	424162	15	NULL	NULL	NULL	NULL	dengue virus infection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results we conclude that Fc gamma RII mediate antibody-dependent enhancement of dengue virus infection in addition to Fc gamma RI .
	manualset3
262569	5	424162	15	NULL	NULL	NULL	NULL	addition	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results we conclude that Fc gamma RII mediate antibody-dependent enhancement of dengue virus infection in addition to Fc gamma RI .
	manualset3
262570	6	424162	15	NULL	NULL	NULL	NULL	Fc gamma RI	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results we conclude that Fc gamma RII mediate antibody-dependent enhancement of dengue virus infection in addition to Fc gamma RI .
	manualset3
262571	1	424163	15	NULL	NULL	NULL	NULL	results	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results we propose that : ( 1 ) the in vitro particulates in EDTA extracts correspond to an observed particulate form of extracellular matrix within the myocardial basement membrane ( MBM ) of mesenchyme-forming regions and ( 2 ) one or more of the proteins in the MBM particulates function to elicit the epithelial-mesenchymal transition .
	manualset3
262572	2	424163	15	NULL	NULL	NULL	NULL	particulates	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results we propose that : ( 1 ) the in vitro particulates in EDTA extracts correspond to an observed particulate form of extracellular matrix within the myocardial basement membrane ( MBM ) of mesenchyme-forming regions and ( 2 ) one or more of the proteins in the MBM particulates function to elicit the epithelial-mesenchymal transition .
	manualset3
262574	3	424163	15	NULL	NULL	NULL	NULL	EDTA extracts	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results we propose that : ( 1 ) the in vitro particulates in EDTA extracts correspond to an observed particulate form of extracellular matrix within the myocardial basement membrane ( MBM ) of mesenchyme-forming regions and ( 2 ) one or more of the proteins in the MBM particulates function to elicit the epithelial-mesenchymal transition .
	manualset3
262577	4	424163	15	NULL	NULL	NULL	NULL	particulate form	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results we propose that : ( 1 ) the in vitro particulates in EDTA extracts correspond to an observed particulate form of extracellular matrix within the myocardial basement membrane ( MBM ) of mesenchyme-forming regions and ( 2 ) one or more of the proteins in the MBM particulates function to elicit the epithelial-mesenchymal transition .
	manualset3
262578	5	424163	15	NULL	NULL	NULL	NULL	extracellular matrix	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results we propose that : ( 1 ) the in vitro particulates in EDTA extracts correspond to an observed particulate form of extracellular matrix within the myocardial basement membrane ( MBM ) of mesenchyme-forming regions and ( 2 ) one or more of the proteins in the MBM particulates function to elicit the epithelial-mesenchymal transition .
	manualset3
262579	6	424163	15	NULL	NULL	NULL	NULL	myocardial basement membrane ( MBM )	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results we propose that : ( 1 ) the in vitro particulates in EDTA extracts correspond to an observed particulate form of extracellular matrix within the myocardial basement membrane ( MBM ) of mesenchyme-forming regions and ( 2 ) one or more of the proteins in the MBM particulates function to elicit the epithelial-mesenchymal transition .
	manualset3
262580	7	424163	15	NULL	NULL	NULL	NULL	mesenchyme-forming regions 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results we propose that : ( 1 ) the in vitro particulates in EDTA extracts correspond to an observed particulate form of extracellular matrix within the myocardial basement membrane ( MBM ) of mesenchyme-forming regions and ( 2 ) one or more of the proteins in the MBM particulates function to elicit the epithelial-mesenchymal transition .
	manualset3
262581	8	424163	15	NULL	NULL	NULL	NULL	one	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results we propose that : ( 1 ) the in vitro particulates in EDTA extracts correspond to an observed particulate form of extracellular matrix within the myocardial basement membrane ( MBM ) of mesenchyme-forming regions and ( 2 ) one or more of the proteins in the MBM particulates function to elicit the epithelial-mesenchymal transition .
	manualset3
262582	9	424163	15	NULL	NULL	NULL	NULL	proteins 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results we propose that : ( 1 ) the in vitro particulates in EDTA extracts correspond to an observed particulate form of extracellular matrix within the myocardial basement membrane ( MBM ) of mesenchyme-forming regions and ( 2 ) one or more of the proteins in the MBM particulates function to elicit the epithelial-mesenchymal transition .
	manualset3
262583	10	424163	15	NULL	NULL	NULL	NULL	MBM particulates	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results we propose that : ( 1 ) the in vitro particulates in EDTA extracts correspond to an observed particulate form of extracellular matrix within the myocardial basement membrane ( MBM ) of mesenchyme-forming regions and ( 2 ) one or more of the proteins in the MBM particulates function to elicit the epithelial-mesenchymal transition .
	manualset3
262584	11	424163	15	NULL	NULL	NULL	NULL	epithelial-mesenchymal transition	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these results we propose that : ( 1 ) the in vitro particulates in EDTA extracts correspond to an observed particulate form of extracellular matrix within the myocardial basement membrane ( MBM ) of mesenchyme-forming regions and ( 2 ) one or more of the proteins in the MBM particulates function to elicit the epithelial-mesenchymal transition .
	manualset3
262585	1	424164	15	NULL	NULL	NULL	NULL	Experimental research 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental research on the genesis of gastroduodenal ulcer induced by antral hyperstimulation ) .
	manualset3
262588	2	424164	15	NULL	NULL	NULL	NULL	genesis of gastroduodenal ulcer	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental research on the genesis of gastroduodenal ulcer induced by antral hyperstimulation ) .
	manualset3
262590	3	424164	15	NULL	NULL	NULL	NULL	antral hyperstimulation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental research on the genesis of gastroduodenal ulcer induced by antral hyperstimulation ) .
	manualset3
262593	1	424165	15	NULL	NULL	NULL	NULL	studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these studies and prediction of intrinsic disorder we propose that the intrinsically unstructured linker stretch preceding the ACP domain might be facilitating movement of ACP domains to various catalytic centers .
	manualset3
262595	2	424165	15	NULL	NULL	NULL	NULL	prediction of intrinsic disorder 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these studies and prediction of intrinsic disorder we propose that the intrinsically unstructured linker stretch preceding the ACP domain might be facilitating movement of ACP domains to various catalytic centers .
	manualset3
262596	3	424165	15	NULL	NULL	NULL	NULL	linker stretch	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these studies and prediction of intrinsic disorder we propose that the intrinsically unstructured linker stretch preceding the ACP domain might be facilitating movement of ACP domains to various catalytic centers .
	manualset3
262603	4	424165	15	NULL	NULL	NULL	NULL	ACP domain	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these studies and prediction of intrinsic disorder we propose that the intrinsically unstructured linker stretch preceding the ACP domain might be facilitating movement of ACP domains to various catalytic centers .
	manualset3
262605	5	424165	15	NULL	NULL	NULL	NULL	movement of ACP domains	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these studies and prediction of intrinsic disorder we propose that the intrinsically unstructured linker stretch preceding the ACP domain might be facilitating movement of ACP domains to various catalytic centers .
	manualset3
262607	6	424165	15	NULL	NULL	NULL	NULL	catalytic centers	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these studies and prediction of intrinsic disorder we propose that the intrinsically unstructured linker stretch preceding the ACP domain might be facilitating movement of ACP domains to various catalytic centers .
	manualset3
262608	1	424166	15	NULL	NULL	NULL	NULL	studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these studies of critical safety factors , the Army has developed and deployed the SPH-4B , a new helmet with improved energy absorption , retention , and stability .
	manualset3
262612	2	424166	15	NULL	NULL	NULL	NULL	safety factors	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these studies of critical safety factors , the Army has developed and deployed the SPH-4B , a new helmet with improved energy absorption , retention , and stability .
	manualset3
262613	3	424166	15	NULL	NULL	NULL	NULL	Army	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these studies of critical safety factors , the Army has developed and deployed the SPH-4B , a new helmet with improved energy absorption , retention , and stability .
	manualset3
262615	4	424166	15	NULL	NULL	NULL	NULL	SPH-4B	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these studies of critical safety factors , the Army has developed and deployed the SPH-4B , a new helmet with improved energy absorption , retention , and stability .
	manualset3
262618	5	424166	15	NULL	NULL	NULL	NULL	helmet 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these studies of critical safety factors , the Army has developed and deployed the SPH-4B , a new helmet with improved energy absorption , retention , and stability .
	manualset3
262620	6	424166	15	NULL	NULL	NULL	NULL	energy absorption	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these studies of critical safety factors , the Army has developed and deployed the SPH-4B , a new helmet with improved energy absorption , retention , and stability .
	manualset3
262622	7	424166	15	NULL	NULL	NULL	NULL	retention 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these studies of critical safety factors , the Army has developed and deployed the SPH-4B , a new helmet with improved energy absorption , retention , and stability .
	manualset3
262623	8	424166	15	NULL	NULL	NULL	NULL	stability	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on these studies of critical safety factors , the Army has developed and deployed the SPH-4B , a new helmet with improved energy absorption , retention , and stability .
	manualset3
262632	1	424167	15	NULL	NULL	NULL	NULL	preliminary study 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on this preliminary study of 45 shoulders , we present a classification of the lesions found in the acute shoulder dislocation .
	manualset3
262633	2	424167	15	NULL	NULL	NULL	NULL	45 shoulders 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on this preliminary study of 45 shoulders , we present a classification of the lesions found in the acute shoulder dislocation .
	manualset3
262634	3	424167	15	NULL	NULL	NULL	NULL	classification	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on this preliminary study of 45 shoulders , we present a classification of the lesions found in the acute shoulder dislocation .
	manualset3
262635	4	424167	15	NULL	NULL	NULL	NULL	lesions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on this preliminary study of 45 shoulders , we present a classification of the lesions found in the acute shoulder dislocation .
	manualset3
262636	5	424167	15	NULL	NULL	NULL	NULL	acute shoulder dislocation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on this preliminary study of 45 shoulders , we present a classification of the lesions found in the acute shoulder dislocation .
	manualset3
262637	1	424168	15	NULL	NULL	NULL	NULL	topographic site of origin	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on topographic site of origin , the GI tract is the single largest component of the biopsy service in this institution .
	manualset3
262638	2	424168	15	NULL	NULL	NULL	NULL	GI tract	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on topographic site of origin , the GI tract is the single largest component of the biopsy service in this institution .
	manualset3
262640	3	424168	15	NULL	NULL	NULL	NULL	component	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on topographic site of origin , the GI tract is the single largest component of the biopsy service in this institution .
	manualset3
262642	4	424168	15	NULL	NULL	NULL	NULL	biopsy service	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on topographic site of origin , the GI tract is the single largest component of the biopsy service in this institution .
	manualset3
262644	5	424168	15	NULL	NULL	NULL	NULL	institution	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based on topographic site of origin , the GI tract is the single largest component of the biopsy service in this institution .
	manualset3
262647	1	424169	15	NULL	NULL	NULL	NULL	clinical signs 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based upon clinical signs related to the laxation effect of senna , the highest dose ( 300 mg/kg/day ) was considered to be a maximum tolerated dose .
	manualset3
262648	2	424169	15	NULL	NULL	NULL	NULL	laxation effect of senna	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based upon clinical signs related to the laxation effect of senna , the highest dose ( 300 mg/kg/day ) was considered to be a maximum tolerated dose .
	manualset3
262650	3	424169	15	NULL	NULL	NULL	NULL	dose ( 300 mg/kg/day ) 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based upon clinical signs related to the laxation effect of senna , the highest dose ( 300 mg/kg/day ) was considered to be a maximum tolerated dose .
	manualset3
262653	4	424169	15	NULL	NULL	NULL	NULL	tolerated dose	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based upon clinical signs related to the laxation effect of senna , the highest dose ( 300 mg/kg/day ) was considered to be a maximum tolerated dose .
	manualset3
262654	1	424170	15	NULL	NULL	NULL	NULL	double-labelling experiments	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based upon double-labelling experiments with antibody against rough endoplasmic reticulum ( RER ) , there is a strong possibility that intra-cellular sites of alpha i2-subunit correspond to association with RER membranes .
	manualset3
262656	2	424170	15	NULL	NULL	NULL	NULL	antibody	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based upon double-labelling experiments with antibody against rough endoplasmic reticulum ( RER ) , there is a strong possibility that intra-cellular sites of alpha i2-subunit correspond to association with RER membranes .
	manualset3
262658	3	424170	15	NULL	NULL	NULL	NULL	rough endoplasmic reticulum ( RER )	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based upon double-labelling experiments with antibody against rough endoplasmic reticulum ( RER ) , there is a strong possibility that intra-cellular sites of alpha i2-subunit correspond to association with RER membranes .
	manualset3
262661	4	424170	15	NULL	NULL	NULL	NULL	possibility	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based upon double-labelling experiments with antibody against rough endoplasmic reticulum ( RER ) , there is a strong possibility that intra-cellular sites of alpha i2-subunit correspond to association with RER membranes .
	manualset3
262663	5	424170	15	NULL	NULL	NULL	NULL	intra-cellular sites of alpha i2-subunit	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based upon double-labelling experiments with antibody against rough endoplasmic reticulum ( RER ) , there is a strong possibility that intra-cellular sites of alpha i2-subunit correspond to association with RER membranes .
	manualset3
262665	6	424170	15	NULL	NULL	NULL	NULL	association	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based upon double-labelling experiments with antibody against rough endoplasmic reticulum ( RER ) , there is a strong possibility that intra-cellular sites of alpha i2-subunit correspond to association with RER membranes .
	manualset3
262666	7	424170	15	NULL	NULL	NULL	NULL	RER membranes	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based upon double-labelling experiments with antibody against rough endoplasmic reticulum ( RER ) , there is a strong possibility that intra-cellular sites of alpha i2-subunit correspond to association with RER membranes .
	manualset3
262669	1	424171	15	NULL	NULL	NULL	NULL	reactions	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based upon the known reactions of nitrogenase and the principles of coordination catalysis , a model of nitrogenase active-centre is proposed .
	manualset3
262670	2	424171	15	NULL	NULL	NULL	NULL	nitrogenase	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based upon the known reactions of nitrogenase and the principles of coordination catalysis , a model of nitrogenase active-centre is proposed .
	manualset3
262671	3	424171	15	NULL	NULL	NULL	NULL	principles of coordination catalysis	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based upon the known reactions of nitrogenase and the principles of coordination catalysis , a model of nitrogenase active-centre is proposed .
	manualset3
262673	4	424171	15	NULL	NULL	NULL	NULL	model of nitrogenase active-centre	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Based upon the known reactions of nitrogenase and the principles of coordination catalysis , a model of nitrogenase active-centre is proposed .
	manualset3
262681	1	424172	15	NULL	NULL	NULL	NULL	Baseline assessment	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline assessment comprised a questionnaire , a medical examination , sampling of blood as well as ad hoc analyses of a range of biomarkers and genetic factors .
	manualset3
262682	2	424172	15	NULL	NULL	NULL	NULL	questionnaire	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline assessment comprised a questionnaire , a medical examination , sampling of blood as well as ad hoc analyses of a range of biomarkers and genetic factors .
	manualset3
262683	3	424172	15	NULL	NULL	NULL	NULL	medical examination 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline assessment comprised a questionnaire , a medical examination , sampling of blood as well as ad hoc analyses of a range of biomarkers and genetic factors .
	manualset3
262684	4	424172	15	NULL	NULL	NULL	NULL	sampling of blood 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline assessment comprised a questionnaire , a medical examination , sampling of blood as well as ad hoc analyses of a range of biomarkers and genetic factors .
	manualset3
262685	5	424172	15	NULL	NULL	NULL	NULL	ad hoc analyses	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline assessment comprised a questionnaire , a medical examination , sampling of blood as well as ad hoc analyses of a range of biomarkers and genetic factors .
	manualset3
262686	6	424172	15	NULL	NULL	NULL	NULL	biomarkers	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline assessment comprised a questionnaire , a medical examination , sampling of blood as well as ad hoc analyses of a range of biomarkers and genetic factors .
	manualset3
262687	7	424172	15	NULL	NULL	NULL	NULL	genetic factors	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline assessment comprised a questionnaire , a medical examination , sampling of blood as well as ad hoc analyses of a range of biomarkers and genetic factors .
	manualset3
262688	1	424173	15	NULL	NULL	NULL	NULL	Baseline characteristics	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline characteristics did not differ among the groups ( mean + / - SEM : 0.37 + / - 0.06 mL/min ) , and tramadol lowered the secretion at the same level in all groups ( 0.15 + / - 0.02 mL/min ) .
	manualset3
262689	2	424173	15	NULL	NULL	NULL	NULL	groups	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline characteristics did not differ among the groups ( mean + / - SEM : 0.37 + / - 0.06 mL/min ) , and tramadol lowered the secretion at the same level in all groups ( 0.15 + / - 0.02 mL/min ) .
	manualset3
262690	3	424173	15	NULL	NULL	NULL	NULL	mean + / - SEM : 0.37 + / - 0.06 mL/min	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline characteristics did not differ among the groups ( mean + / - SEM : 0.37 + / - 0.06 mL/min ) , and tramadol lowered the secretion at the same level in all groups ( 0.15 + / - 0.02 mL/min ) .
	manualset3
262691	4	424173	15	NULL	NULL	NULL	NULL	tramadol 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline characteristics did not differ among the groups ( mean + / - SEM : 0.37 + / - 0.06 mL/min ) , and tramadol lowered the secretion at the same level in all groups ( 0.15 + / - 0.02 mL/min ) .
	manualset3
262692	5	424173	15	NULL	NULL	NULL	NULL	secretion 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline characteristics did not differ among the groups ( mean + / - SEM : 0.37 + / - 0.06 mL/min ) , and tramadol lowered the secretion at the same level in all groups ( 0.15 + / - 0.02 mL/min ) .
	manualset3
262693	6	424173	15	NULL	NULL	NULL	NULL	level	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline characteristics did not differ among the groups ( mean + / - SEM : 0.37 + / - 0.06 mL/min ) , and tramadol lowered the secretion at the same level in all groups ( 0.15 + / - 0.02 mL/min ) .
	manualset3
262694	7	424173	15	NULL	NULL	NULL	NULL	groups	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline characteristics did not differ among the groups ( mean + / - SEM : 0.37 + / - 0.06 mL/min ) , and tramadol lowered the secretion at the same level in all groups ( 0.15 + / - 0.02 mL/min ) .
	manualset3
262695	8	424173	15	NULL	NULL	NULL	NULL	0.15 + / - 0.02 mL/min 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline characteristics did not differ among the groups ( mean + / - SEM : 0.37 + / - 0.06 mL/min ) , and tramadol lowered the secretion at the same level in all groups ( 0.15 + / - 0.02 mL/min ) .
	manualset3
262792	1	424174	15	NULL	NULL	NULL	NULL	Baseline data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline data from 285 community-dwelling elders with a research classification of dementia enrolled in the observational Memory and Medical Care Study were analyzed .
	manualset3
262793	2	424174	15	NULL	NULL	NULL	NULL	285	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline data from 285 community-dwelling elders with a research classification of dementia enrolled in the observational Memory and Medical Care Study were analyzed .
	manualset3
262794	3	424174	15	NULL	NULL	NULL	NULL	community-dwelling elders	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline data from 285 community-dwelling elders with a research classification of dementia enrolled in the observational Memory and Medical Care Study were analyzed .
	manualset3
262795	4	424174	15	NULL	NULL	NULL	NULL	research classification 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline data from 285 community-dwelling elders with a research classification of dementia enrolled in the observational Memory and Medical Care Study were analyzed .
	manualset3
262796	5	424174	15	NULL	NULL	NULL	NULL	dementia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline data from 285 community-dwelling elders with a research classification of dementia enrolled in the observational Memory and Medical Care Study were analyzed .
	manualset3
262797	6	424174	15	NULL	NULL	NULL	NULL	observational Memory Study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline data from 285 community-dwelling elders with a research classification of dementia enrolled in the observational Memory and Medical Care Study were analyzed .
	manualset3
262798	7	424174	15	NULL	NULL	NULL	NULL	Medical Care Study 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline data from 285 community-dwelling elders with a research classification of dementia enrolled in the observational Memory and Medical Care Study were analyzed .
	manualset3
262799	1	424175	15	NULL	NULL	NULL	NULL	Experimental studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental studies of the dynamo-muscular effect of adrenoxyl ; a monosemicarbazone derivative of adrenochrome ) .
	manualset3
262800	2	424175	15	NULL	NULL	NULL	NULL	dynamo-muscular effect 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental studies of the dynamo-muscular effect of adrenoxyl ; a monosemicarbazone derivative of adrenochrome ) .
	manualset3
262801	3	424175	15	NULL	NULL	NULL	NULL	adrenoxyl	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental studies of the dynamo-muscular effect of adrenoxyl ; a monosemicarbazone derivative of adrenochrome ) .
	manualset3
262802	4	424175	15	NULL	NULL	NULL	NULL	monosemicarbazone derivative	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental studies of the dynamo-muscular effect of adrenoxyl ; a monosemicarbazone derivative of adrenochrome ) .
	manualset3
262803	5	424175	15	NULL	NULL	NULL	NULL	adrenochrome	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental studies of the dynamo-muscular effect of adrenoxyl ; a monosemicarbazone derivative of adrenochrome ) .
	manualset3
262804	1	424176	15	NULL	NULL	NULL	NULL	Baseline function 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline function was normal and no change occurred following diuresis .
	manualset3
262805	2	424176	15	NULL	NULL	NULL	NULL	change	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline function was normal and no change occurred following diuresis .
	manualset3
262806	3	424176	15	NULL	NULL	NULL	NULL	diuresis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline function was normal and no change occurred following diuresis .
	manualset3
262807	1	424177	15	NULL	NULL	NULL	NULL	Baseline values	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline values of the micturition volume and frequency of nine male and 10 female SD adult rats were measured over a 24-hour time period .
	manualset3
262808	2	424177	15	NULL	NULL	NULL	NULL	micturition volume 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline values of the micturition volume and frequency of nine male and 10 female SD adult rats were measured over a 24-hour time period .
	manualset3
262809	3	424177	15	NULL	NULL	NULL	NULL	frequency	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline values of the micturition volume and frequency of nine male and 10 female SD adult rats were measured over a 24-hour time period .
	manualset3
262810	4	424177	15	NULL	NULL	NULL	NULL	nine male SD adult rats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline values of the micturition volume and frequency of nine male and 10 female SD adult rats were measured over a 24-hour time period .
	manualset3
262811	5	424177	15	NULL	NULL	NULL	NULL	10 female SD adult rats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline values of the micturition volume and frequency of nine male and 10 female SD adult rats were measured over a 24-hour time period .
	manualset3
262812	6	424177	15	NULL	NULL	NULL	NULL	24-hour time period 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Baseline values of the micturition volume and frequency of nine male and 10 female SD adult rats were measured over a 24-hour time period .
	manualset3
262813	1	424178	15	NULL	NULL	NULL	NULL	Basement membrane collagen	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basement membrane collagen requirements for attachment and growth of mammary epithelium .
	manualset3
263415	2	424178	15	NULL	NULL	NULL	NULL	requirements 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basement membrane collagen requirements for attachment and growth of mammary epithelium .
	manualset3
263416	3	424178	15	NULL	NULL	NULL	NULL	attachment	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basement membrane collagen requirements for attachment and growth of mammary epithelium .
	manualset3
263417	4	424178	15	NULL	NULL	NULL	NULL	growth of mammary epithelium	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basement membrane collagen requirements for attachment and growth of mammary epithelium .
	manualset3
263418	1	424179	15	NULL	NULL	NULL	NULL	Basement membranes ( BM ) 	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basement membranes ( BM ) are elements of the extracellular matrix that are essential for growth and differentiation of tissues .
	manualset3
263419	2	424179	15	NULL	NULL	NULL	NULL	 elements	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basement membranes ( BM ) are elements of the extracellular matrix that are essential for growth and differentiation of tissues .
	manualset3
263420	3	424179	15	NULL	NULL	NULL	NULL	extracellular matrix	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basement membranes ( BM ) are elements of the extracellular matrix that are essential for growth and differentiation of tissues .
	manualset3
263421	4	424179	15	NULL	NULL	NULL	NULL	growth 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basement membranes ( BM ) are elements of the extracellular matrix that are essential for growth and differentiation of tissues .
	manualset3
263422	5	424179	15	NULL	NULL	NULL	NULL	differentiation of tissues 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basement membranes ( BM ) are elements of the extracellular matrix that are essential for growth and differentiation of tissues .
	manualset3
263423	1	424180	15	NULL	NULL	NULL	NULL	Basic sampling method 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basic sampling method adopted was Probability Proportional to Size ( PPS ) sampling .
	manualset3
263424	2	424180	15	NULL	NULL	NULL	NULL	Probability Proportional to Size ( PPS ) sampling 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basic sampling method adopted was Probability Proportional to Size ( PPS ) sampling .
	manualset3
263425	1	424181	15	NULL	NULL	NULL	NULL	two	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basing on two own observations , swelling of the Achilles tendon by xanthomas in familial hypercholesterolemia is described .
	manualset3
263426	2	424181	15	NULL	NULL	NULL	NULL	observations	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basing on two own observations , swelling of the Achilles tendon by xanthomas in familial hypercholesterolemia is described .
	manualset3
263427	3	424181	15	NULL	NULL	NULL	NULL	swelling of the Achilles tendon	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basing on two own observations , swelling of the Achilles tendon by xanthomas in familial hypercholesterolemia is described .
	manualset3
263428	4	424181	15	NULL	NULL	NULL	NULL	xanthomas 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basing on two own observations , swelling of the Achilles tendon by xanthomas in familial hypercholesterolemia is described .
	manualset3
263429	5	424181	15	NULL	NULL	NULL	NULL	familial hypercholesterolemia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basing on two own observations , swelling of the Achilles tendon by xanthomas in familial hypercholesterolemia is described .
	manualset3
263430	1	424182	15	NULL	NULL	NULL	NULL	Basolateral to apical transport	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basolateral to apical transport did not depend upon determinants in the cytoplasmic domain .
	manualset3
263431	2	424182	15	NULL	NULL	NULL	NULL	determinants	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basolateral to apical transport did not depend upon determinants in the cytoplasmic domain .
	manualset3
263432	3	424182	15	NULL	NULL	NULL	NULL	cytoplasmic domain 	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Basolateral to apical transport did not depend upon determinants in the cytoplasmic domain .
	manualset3
263433	1	424183	15	NULL	NULL	NULL	NULL	Switching	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( 1 ) Switching from a cis to a trans isomer of a monounsaturated FA chain in phosphatidylcholine ( PC ) increased - activity , did not affect A ( 42 ) : A ( 40 ) ratios , but decreased the ratio of long ( 42 ) versus short ( 41 ) A peptides .
	manualset3
263434	2	424183	15	NULL	NULL	NULL	NULL	cis isomer 	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( 1 ) Switching from a cis to a trans isomer of a monounsaturated FA chain in phosphatidylcholine ( PC ) increased - activity , did not affect A ( 42 ) : A ( 40 ) ratios , but decreased the ratio of long ( 42 ) versus short ( 41 ) A peptides .
	manualset3
263435	3	424183	15	NULL	NULL	NULL	NULL	trans isomer	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( 1 ) Switching from a cis to a trans isomer of a monounsaturated FA chain in phosphatidylcholine ( PC ) increased - activity , did not affect A ( 42 ) : A ( 40 ) ratios , but decreased the ratio of long ( 42 ) versus short ( 41 ) A peptides .
	manualset3
263436	4	424183	15	NULL	NULL	NULL	NULL	monounsaturated FA chain	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( 1 ) Switching from a cis to a trans isomer of a monounsaturated FA chain in phosphatidylcholine ( PC ) increased - activity , did not affect A ( 42 ) : A ( 40 ) ratios , but decreased the ratio of long ( 42 ) versus short ( 41 ) A peptides .
	manualset3
263437	5	424183	15	NULL	NULL	NULL	NULL	phosphatidylcholine ( PC ) 	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( 1 ) Switching from a cis to a trans isomer of a monounsaturated FA chain in phosphatidylcholine ( PC ) increased - activity , did not affect A ( 42 ) : A ( 40 ) ratios , but decreased the ratio of long ( 42 ) versus short ( 41 ) A peptides .
	manualset3
263438	6	424183	15	NULL	NULL	NULL	NULL	activity 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( 1 ) Switching from a cis to a trans isomer of a monounsaturated FA chain in phosphatidylcholine ( PC ) increased - activity , did not affect A ( 42 ) : A ( 40 ) ratios , but decreased the ratio of long ( 42 ) versus short ( 41 ) A peptides .
	manualset3
263439	7	424183	15	NULL	NULL	NULL	NULL	affect	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( 1 ) Switching from a cis to a trans isomer of a monounsaturated FA chain in phosphatidylcholine ( PC ) increased - activity , did not affect A ( 42 ) : A ( 40 ) ratios , but decreased the ratio of long ( 42 ) versus short ( 41 ) A peptides .
	manualset3
263440	8	424183	15	NULL	NULL	NULL	NULL	A ( 42 ) : A ( 40 ) ratios	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( 1 ) Switching from a cis to a trans isomer of a monounsaturated FA chain in phosphatidylcholine ( PC ) increased - activity , did not affect A ( 42 ) : A ( 40 ) ratios , but decreased the ratio of long ( 42 ) versus short ( 41 ) A peptides .
	manualset3
263441	9	424183	15	NULL	NULL	NULL	NULL	ratio 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( 1 ) Switching from a cis to a trans isomer of a monounsaturated FA chain in phosphatidylcholine ( PC ) increased - activity , did not affect A ( 42 ) : A ( 40 ) ratios , but decreased the ratio of long ( 42 ) versus short ( 41 ) A peptides .
	manualset3
263442	10	424183	15	NULL	NULL	NULL	NULL	long ( 42 ) peptides	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( 1 ) Switching from a cis to a trans isomer of a monounsaturated FA chain in phosphatidylcholine ( PC ) increased - activity , did not affect A ( 42 ) : A ( 40 ) ratios , but decreased the ratio of long ( 42 ) versus short ( 41 ) A peptides .
	manualset3
263443	11	424183	15	NULL	NULL	NULL	NULL	short ( 41 ) A peptides	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( 1 ) Switching from a cis to a trans isomer of a monounsaturated FA chain in phosphatidylcholine ( PC ) increased - activity , did not affect A ( 42 ) : A ( 40 ) ratios , but decreased the ratio of long ( 42 ) versus short ( 41 ) A peptides .
	manualset3
263444	1	424184	15	NULL	NULL	NULL	NULL	device	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( A device for measuring nonuniformity of the dose field of ionizing radiation ) .
	manualset3
263445	2	424184	15	NULL	NULL	NULL	NULL	nonuniformity	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( A device for measuring nonuniformity of the dose field of ionizing radiation ) .
	manualset3
263446	3	424184	15	NULL	NULL	NULL	NULL	dose field 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( A device for measuring nonuniformity of the dose field of ionizing radiation ) .
	manualset3
263447	4	424184	15	NULL	NULL	NULL	NULL	ionizing radiation 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( A device for measuring nonuniformity of the dose field of ionizing radiation ) .
	manualset3
263448	1	424185	15	NULL	NULL	NULL	NULL	Experimental studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental studies on the amount of vitamin B2 in the blood and organs of rabbits with liver diseases .
	manualset3
263449	2	424185	15	NULL	NULL	NULL	NULL	amount of vitamin B2	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental studies on the amount of vitamin B2 in the blood and organs of rabbits with liver diseases .
	manualset3
263450	3	424185	15	NULL	NULL	NULL	NULL	 blood	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental studies on the amount of vitamin B2 in the blood and organs of rabbits with liver diseases .
	manualset3
263451	4	424185	15	NULL	NULL	NULL	NULL	organs	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental studies on the amount of vitamin B2 in the blood and organs of rabbits with liver diseases .
	manualset3
263452	5	424185	15	NULL	NULL	NULL	NULL	rabbits	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental studies on the amount of vitamin B2 in the blood and organs of rabbits with liver diseases .
	manualset3
263453	6	424185	15	NULL	NULL	NULL	NULL	liver diseases 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental studies on the amount of vitamin B2 in the blood and organs of rabbits with liver diseases .
	manualset3
263454	1	424186	15	NULL	NULL	NULL	NULL	Bath application	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bath application of ( RS ) -2 , 3 , 4 , 5 - tetrahydro-7 , 8 - dihydroxy-1-phenyl-1H-3-benzazepine hydrochloride ( SKF-38393 ) , a dopaminergic D1-class receptor agonist , increased evoked EPSCs by approximately 30 % whereas the D2-class receptor agonist , trans - ( - ) -4 aR-4 , 4 a , 5 , 6 , 7 , 8 , 8a , 9-octahydro-5-propyl-1H-pyrazolo ( 3 , 4-g ) quinoline ( quinpirole ) , reduced EPSCs by approximately 25 % .
	manualset3
263455	2	424186	15	NULL	NULL	NULL	NULL	( RS ) -2 , 3 , 4 , 5 - tetrahydro-7 , 8 - dihydroxy-1-phenyl-1H-3-benzazepine hydrochloride ( SKF-38393 )	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bath application of ( RS ) -2 , 3 , 4 , 5 - tetrahydro-7 , 8 - dihydroxy-1-phenyl-1H-3-benzazepine hydrochloride ( SKF-38393 ) , a dopaminergic D1-class receptor agonist , increased evoked EPSCs by approximately 30 % whereas the D2-class receptor agonist , trans - ( - ) -4 aR-4 , 4 a , 5 , 6 , 7 , 8 , 8a , 9-octahydro-5-propyl-1H-pyrazolo ( 3 , 4-g ) quinoline ( quinpirole ) , reduced EPSCs by approximately 25 % .
	manualset3
263456	3	424186	15	NULL	NULL	NULL	NULL	dopaminergic D1-class receptor agonist	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bath application of ( RS ) -2 , 3 , 4 , 5 - tetrahydro-7 , 8 - dihydroxy-1-phenyl-1H-3-benzazepine hydrochloride ( SKF-38393 ) , a dopaminergic D1-class receptor agonist , increased evoked EPSCs by approximately 30 % whereas the D2-class receptor agonist , trans - ( - ) -4 aR-4 , 4 a , 5 , 6 , 7 , 8 , 8a , 9-octahydro-5-propyl-1H-pyrazolo ( 3 , 4-g ) quinoline ( quinpirole ) , reduced EPSCs by approximately 25 % .
	manualset3
263457	4	424186	15	NULL	NULL	NULL	NULL	EPSCs	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bath application of ( RS ) -2 , 3 , 4 , 5 - tetrahydro-7 , 8 - dihydroxy-1-phenyl-1H-3-benzazepine hydrochloride ( SKF-38393 ) , a dopaminergic D1-class receptor agonist , increased evoked EPSCs by approximately 30 % whereas the D2-class receptor agonist , trans - ( - ) -4 aR-4 , 4 a , 5 , 6 , 7 , 8 , 8a , 9-octahydro-5-propyl-1H-pyrazolo ( 3 , 4-g ) quinoline ( quinpirole ) , reduced EPSCs by approximately 25 % .
	manualset3
263458	5	424186	15	NULL	NULL	NULL	NULL	30 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bath application of ( RS ) -2 , 3 , 4 , 5 - tetrahydro-7 , 8 - dihydroxy-1-phenyl-1H-3-benzazepine hydrochloride ( SKF-38393 ) , a dopaminergic D1-class receptor agonist , increased evoked EPSCs by approximately 30 % whereas the D2-class receptor agonist , trans - ( - ) -4 aR-4 , 4 a , 5 , 6 , 7 , 8 , 8a , 9-octahydro-5-propyl-1H-pyrazolo ( 3 , 4-g ) quinoline ( quinpirole ) , reduced EPSCs by approximately 25 % .
	manualset3
263459	6	424186	15	NULL	NULL	NULL	NULL	D2-class receptor agonist	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bath application of ( RS ) -2 , 3 , 4 , 5 - tetrahydro-7 , 8 - dihydroxy-1-phenyl-1H-3-benzazepine hydrochloride ( SKF-38393 ) , a dopaminergic D1-class receptor agonist , increased evoked EPSCs by approximately 30 % whereas the D2-class receptor agonist , trans - ( - ) -4 aR-4 , 4 a , 5 , 6 , 7 , 8 , 8a , 9-octahydro-5-propyl-1H-pyrazolo ( 3 , 4-g ) quinoline ( quinpirole ) , reduced EPSCs by approximately 25 % .
	manualset3
263460	7	424186	15	NULL	NULL	NULL	NULL	trans - ( - ) -4 aR-4 , 4 a , 5 , 6 , 7 , 8 , 8a , 9-octahydro-5-propyl-1H-pyrazolo ( 3 , 4-g ) quinoline ( quinpirole ) 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bath application of ( RS ) -2 , 3 , 4 , 5 - tetrahydro-7 , 8 - dihydroxy-1-phenyl-1H-3-benzazepine hydrochloride ( SKF-38393 ) , a dopaminergic D1-class receptor agonist , increased evoked EPSCs by approximately 30 % whereas the D2-class receptor agonist , trans - ( - ) -4 aR-4 , 4 a , 5 , 6 , 7 , 8 , 8a , 9-octahydro-5-propyl-1H-pyrazolo ( 3 , 4-g ) quinoline ( quinpirole ) , reduced EPSCs by approximately 25 % .
	manualset3
263461	8	424186	15	NULL	NULL	NULL	NULL	EPSCs 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bath application of ( RS ) -2 , 3 , 4 , 5 - tetrahydro-7 , 8 - dihydroxy-1-phenyl-1H-3-benzazepine hydrochloride ( SKF-38393 ) , a dopaminergic D1-class receptor agonist , increased evoked EPSCs by approximately 30 % whereas the D2-class receptor agonist , trans - ( - ) -4 aR-4 , 4 a , 5 , 6 , 7 , 8 , 8a , 9-octahydro-5-propyl-1H-pyrazolo ( 3 , 4-g ) quinoline ( quinpirole ) , reduced EPSCs by approximately 25 % .
	manualset3
263462	9	424186	15	NULL	NULL	NULL	NULL	25 % 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bath application of ( RS ) -2 , 3 , 4 , 5 - tetrahydro-7 , 8 - dihydroxy-1-phenyl-1H-3-benzazepine hydrochloride ( SKF-38393 ) , a dopaminergic D1-class receptor agonist , increased evoked EPSCs by approximately 30 % whereas the D2-class receptor agonist , trans - ( - ) -4 aR-4 , 4 a , 5 , 6 , 7 , 8 , 8a , 9-octahydro-5-propyl-1H-pyrazolo ( 3 , 4-g ) quinoline ( quinpirole ) , reduced EPSCs by approximately 25 % .
	manualset3
263463	1	424187	15	NULL	NULL	NULL	NULL	Bath application 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bath application of glycine and its agonist beta-alanine further confirmed the transitory depolarizing action of glycine in the auditory brainstem .
	manualset3
263464	2	424187	15	NULL	NULL	NULL	NULL	glycine	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bath application of glycine and its agonist beta-alanine further confirmed the transitory depolarizing action of glycine in the auditory brainstem .
	manualset3
263465	3	424187	15	NULL	NULL	NULL	NULL	agonist	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bath application of glycine and its agonist beta-alanine further confirmed the transitory depolarizing action of glycine in the auditory brainstem .
	manualset3
263466	4	424187	15	NULL	NULL	NULL	NULL	beta-alanine	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bath application of glycine and its agonist beta-alanine further confirmed the transitory depolarizing action of glycine in the auditory brainstem .
	manualset3
263467	5	424187	15	NULL	NULL	NULL	NULL	depolarizing action 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bath application of glycine and its agonist beta-alanine further confirmed the transitory depolarizing action of glycine in the auditory brainstem .
	manualset3
263468	6	424187	15	NULL	NULL	NULL	NULL	glycine	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bath application of glycine and its agonist beta-alanine further confirmed the transitory depolarizing action of glycine in the auditory brainstem .
	manualset3
263469	7	424187	15	NULL	NULL	NULL	NULL	auditory brainstem 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bath application of glycine and its agonist beta-alanine further confirmed the transitory depolarizing action of glycine in the auditory brainstem .
	manualset3
263470	1	424188	15	NULL	NULL	NULL	NULL	Bath application 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bath application of serotonin also induced transient increase in ciliary transport rate , followed by inhibition of ciliary activity up to its full cessation in some areas of isolated foregut .
	manualset3
263471	2	424188	15	NULL	NULL	NULL	NULL	serotonin	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bath application of serotonin also induced transient increase in ciliary transport rate , followed by inhibition of ciliary activity up to its full cessation in some areas of isolated foregut .
	manualset3
263472	3	424188	15	NULL	NULL	NULL	NULL	increase	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bath application of serotonin also induced transient increase in ciliary transport rate , followed by inhibition of ciliary activity up to its full cessation in some areas of isolated foregut .
	manualset3
263473	4	424188	15	NULL	NULL	NULL	NULL	ciliary transport rate	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bath application of serotonin also induced transient increase in ciliary transport rate , followed by inhibition of ciliary activity up to its full cessation in some areas of isolated foregut .
	manualset3
263474	5	424188	15	NULL	NULL	NULL	NULL	inhibition of ciliary activity 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bath application of serotonin also induced transient increase in ciliary transport rate , followed by inhibition of ciliary activity up to its full cessation in some areas of isolated foregut .
	manualset3
263475	6	424188	15	NULL	NULL	NULL	NULL	cessation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bath application of serotonin also induced transient increase in ciliary transport rate , followed by inhibition of ciliary activity up to its full cessation in some areas of isolated foregut .
	manualset3
263476	7	424188	15	NULL	NULL	NULL	NULL	areas of isolated foregut	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bath application of serotonin also induced transient increase in ciliary transport rate , followed by inhibition of ciliary activity up to its full cessation in some areas of isolated foregut .
	manualset3
263477	1	424189	15	NULL	NULL	NULL	NULL	Bayesian estimation 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bayesian estimation of the probability of asbestos exposure from lung fiber counts .
	manualset3
263478	2	424189	15	NULL	NULL	NULL	NULL	probability	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bayesian estimation of the probability of asbestos exposure from lung fiber counts .
	manualset3
263479	3	424189	15	NULL	NULL	NULL	NULL	asbestos exposure	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bayesian estimation of the probability of asbestos exposure from lung fiber counts .
	manualset3
263480	4	424189	15	NULL	NULL	NULL	NULL	lung fiber counts	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bayesian estimation of the probability of asbestos exposure from lung fiber counts .
	manualset3
263481	1	424190	15	NULL	NULL	NULL	NULL	Bayesian methods of estimation 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bayesian methods of estimation are used and their value is discussed .
	manualset3
263482	2	424190	15	NULL	NULL	NULL	NULL	value	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bayesian methods of estimation are used and their value is discussed .
	manualset3
263483	1	424191	15	NULL	NULL	NULL	NULL	Bayesian non-response models 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bayesian non-response models for categorical data from small areas : an application to BMD and age .
	manualset3
263484	2	424191	15	NULL	NULL	NULL	NULL	categorical data 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bayesian non-response models for categorical data from small areas : an application to BMD and age .
	manualset3
263485	3	424191	15	NULL	NULL	NULL	NULL	areas	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bayesian non-response models for categorical data from small areas : an application to BMD and age .
	manualset3
263486	4	424191	15	NULL	NULL	NULL	NULL	application	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bayesian non-response models for categorical data from small areas : an application to BMD and age .
	manualset3
263487	5	424191	15	NULL	NULL	NULL	NULL	BMD	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bayesian non-response models for categorical data from small areas : an application to BMD and age .
	manualset3
263488	6	424191	15	NULL	NULL	NULL	NULL	age	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bayesian non-response models for categorical data from small areas : an application to BMD and age .
	manualset3
263489	1	424192	15	NULL	NULL	NULL	NULL	BbPlgl 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BbPlgl was also able to auto-activate at neutral and alkaline pH at 4 degrees C without the addition of uPA , and the activation was accelerated by addition of human uPA .
	manualset3
263490	2	424192	15	NULL	NULL	NULL	NULL	auto-activate	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BbPlgl was also able to auto-activate at neutral and alkaline pH at 4 degrees C without the addition of uPA , and the activation was accelerated by addition of human uPA .
	manualset3
263491	3	424192	15	NULL	NULL	NULL	NULL	neutral pH	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BbPlgl was also able to auto-activate at neutral and alkaline pH at 4 degrees C without the addition of uPA , and the activation was accelerated by addition of human uPA .
	manualset3
263492	4	424192	15	NULL	NULL	NULL	NULL	alkaline pH	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BbPlgl was also able to auto-activate at neutral and alkaline pH at 4 degrees C without the addition of uPA , and the activation was accelerated by addition of human uPA .
	manualset3
263493	5	424192	15	NULL	NULL	NULL	NULL	4 degrees C	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BbPlgl was also able to auto-activate at neutral and alkaline pH at 4 degrees C without the addition of uPA , and the activation was accelerated by addition of human uPA .
	manualset3
263494	6	424192	15	NULL	NULL	NULL	NULL	addition	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BbPlgl was also able to auto-activate at neutral and alkaline pH at 4 degrees C without the addition of uPA , and the activation was accelerated by addition of human uPA .
	manualset3
263495	7	424192	15	NULL	NULL	NULL	NULL	uPA	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BbPlgl was also able to auto-activate at neutral and alkaline pH at 4 degrees C without the addition of uPA , and the activation was accelerated by addition of human uPA .
	manualset3
263496	8	424192	15	NULL	NULL	NULL	NULL	activation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BbPlgl was also able to auto-activate at neutral and alkaline pH at 4 degrees C without the addition of uPA , and the activation was accelerated by addition of human uPA .
	manualset3
263497	9	424192	15	NULL	NULL	NULL	NULL	addition	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BbPlgl was also able to auto-activate at neutral and alkaline pH at 4 degrees C without the addition of uPA , and the activation was accelerated by addition of human uPA .
	manualset3
263498	10	424192	15	NULL	NULL	NULL	NULL	human uPA 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BbPlgl was also able to auto-activate at neutral and alkaline pH at 4 degrees C without the addition of uPA , and the activation was accelerated by addition of human uPA .
	manualset3
263499	1	424193	15	NULL	NULL	NULL	NULL	Bcl-xES	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bcl-xES had a preventive effect on cell death induced by tumor necrosis factor-alpha and various concentrations of anticancer drugs , including camptothecin , etoposide and cisplatin .
	manualset3
263500	2	424193	15	NULL	NULL	NULL	NULL	preventive effect	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bcl-xES had a preventive effect on cell death induced by tumor necrosis factor-alpha and various concentrations of anticancer drugs , including camptothecin , etoposide and cisplatin .
	manualset3
263501	3	424193	15	NULL	NULL	NULL	NULL	cell death	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bcl-xES had a preventive effect on cell death induced by tumor necrosis factor-alpha and various concentrations of anticancer drugs , including camptothecin , etoposide and cisplatin .
	manualset3
263502	4	424193	15	NULL	NULL	NULL	NULL	tumor necrosis factor-alpha	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bcl-xES had a preventive effect on cell death induced by tumor necrosis factor-alpha and various concentrations of anticancer drugs , including camptothecin , etoposide and cisplatin .
	manualset3
263503	5	424193	15	NULL	NULL	NULL	NULL	concentrations	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bcl-xES had a preventive effect on cell death induced by tumor necrosis factor-alpha and various concentrations of anticancer drugs , including camptothecin , etoposide and cisplatin .
	manualset3
263504	6	424193	15	NULL	NULL	NULL	NULL	anticancer drugs 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bcl-xES had a preventive effect on cell death induced by tumor necrosis factor-alpha and various concentrations of anticancer drugs , including camptothecin , etoposide and cisplatin .
	manualset3
263505	7	424193	15	NULL	NULL	NULL	NULL	camptothecin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bcl-xES had a preventive effect on cell death induced by tumor necrosis factor-alpha and various concentrations of anticancer drugs , including camptothecin , etoposide and cisplatin .
	manualset3
263506	8	424193	15	NULL	NULL	NULL	NULL	etoposide	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bcl-xES had a preventive effect on cell death induced by tumor necrosis factor-alpha and various concentrations of anticancer drugs , including camptothecin , etoposide and cisplatin .
	manualset3
263507	9	424193	15	NULL	NULL	NULL	NULL	cisplatin 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bcl-xES had a preventive effect on cell death induced by tumor necrosis factor-alpha and various concentrations of anticancer drugs , including camptothecin , etoposide and cisplatin .
	manualset3
263508	1	424194	15	NULL	NULL	NULL	NULL	Beat-to-beat R-R intervals	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Beat-to-beat R-R intervals ( RRI , i.e. , HRV ) , systolic blood pressure ( SBP ) , and instantaneous lung volume were continuously monitored throughout these periods .
	manualset3
263509	2	424194	15	NULL	NULL	NULL	NULL	RRI 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Beat-to-beat R-R intervals ( RRI , i.e. , HRV ) , systolic blood pressure ( SBP ) , and instantaneous lung volume were continuously monitored throughout these periods .
	manualset3
263510	3	424194	15	NULL	NULL	NULL	NULL	HRV	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Beat-to-beat R-R intervals ( RRI , i.e. , HRV ) , systolic blood pressure ( SBP ) , and instantaneous lung volume were continuously monitored throughout these periods .
	manualset3
263511	4	424194	15	NULL	NULL	NULL	NULL	systolic blood pressure ( SBP ) 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Beat-to-beat R-R intervals ( RRI , i.e. , HRV ) , systolic blood pressure ( SBP ) , and instantaneous lung volume were continuously monitored throughout these periods .
	manualset3
263512	5	424194	15	NULL	NULL	NULL	NULL	instantaneous lung volume	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Beat-to-beat R-R intervals ( RRI , i.e. , HRV ) , systolic blood pressure ( SBP ) , and instantaneous lung volume were continuously monitored throughout these periods .
	manualset3
263513	6	424194	15	NULL	NULL	NULL	NULL	periods 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Beat-to-beat R-R intervals ( RRI , i.e. , HRV ) , systolic blood pressure ( SBP ) , and instantaneous lung volume were continuously monitored throughout these periods .
	manualset3
263514	1	424195	15	NULL	NULL	NULL	NULL	Experimental studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental studies on tuberculin hypersensitivity -- immunological significance of leucocyte migration inhibitory factor ( LIF ) and macrophage migration inhibitory factor ( MIF ) ( author 's transl ) ) .
	manualset3
263515	2	424195	15	NULL	NULL	NULL	NULL	tuberculin hypersensitivity 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental studies on tuberculin hypersensitivity -- immunological significance of leucocyte migration inhibitory factor ( LIF ) and macrophage migration inhibitory factor ( MIF ) ( author 's transl ) ) .
	manualset3
263516	3	424195	15	NULL	NULL	NULL	NULL	immunological significance 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental studies on tuberculin hypersensitivity -- immunological significance of leucocyte migration inhibitory factor ( LIF ) and macrophage migration inhibitory factor ( MIF ) ( author 's transl ) ) .
	manualset3
263531	4	424195	15	NULL	NULL	NULL	NULL	leucocyte migration inhibitory factor ( LIF ) 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental studies on tuberculin hypersensitivity -- immunological significance of leucocyte migration inhibitory factor ( LIF ) and macrophage migration inhibitory factor ( MIF ) ( author 's transl ) ) .
	manualset3
263532	5	424195	15	NULL	NULL	NULL	NULL	macrophage migration inhibitory factor ( MIF ) 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental studies on tuberculin hypersensitivity -- immunological significance of leucocyte migration inhibitory factor ( LIF ) and macrophage migration inhibitory factor ( MIF ) ( author 's transl ) ) .
	manualset3
263533	6	424195	15	NULL	NULL	NULL	NULL	author 's transl 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental studies on tuberculin hypersensitivity -- immunological significance of leucocyte migration inhibitory factor ( LIF ) and macrophage migration inhibitory factor ( MIF ) ( author 's transl ) ) .
	manualset3
263534	1	424196	15	NULL	NULL	NULL	NULL	IV-spectrin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because IV-spectrin does not interact with KCNQ2/3 subunits , it is suspected that IV-spectrin regulates the distribution of KCNQ2/3 subunits in axonal subdomains via regulatory partners .
	manualset3
263535	2	424196	15	NULL	NULL	NULL	NULL	KCNQ2/3 subunits	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because IV-spectrin does not interact with KCNQ2/3 subunits , it is suspected that IV-spectrin regulates the distribution of KCNQ2/3 subunits in axonal subdomains via regulatory partners .
	manualset3
263536	3	424196	15	NULL	NULL	NULL	NULL	IV-spectrin 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because IV-spectrin does not interact with KCNQ2/3 subunits , it is suspected that IV-spectrin regulates the distribution of KCNQ2/3 subunits in axonal subdomains via regulatory partners .
	manualset3
263537	4	424196	15	NULL	NULL	NULL	NULL	distribution of KCNQ2/3 subunits	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because IV-spectrin does not interact with KCNQ2/3 subunits , it is suspected that IV-spectrin regulates the distribution of KCNQ2/3 subunits in axonal subdomains via regulatory partners .
	manualset3
263538	5	424196	15	NULL	NULL	NULL	NULL	axonal subdomains 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because IV-spectrin does not interact with KCNQ2/3 subunits , it is suspected that IV-spectrin regulates the distribution of KCNQ2/3 subunits in axonal subdomains via regulatory partners .
	manualset3
263539	6	424196	15	NULL	NULL	NULL	NULL	regulatory partners	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because IV-spectrin does not interact with KCNQ2/3 subunits , it is suspected that IV-spectrin regulates the distribution of KCNQ2/3 subunits in axonal subdomains via regulatory partners .
	manualset3
263540	1	424197	15	NULL	NULL	NULL	NULL	PCBD-NAC	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because PCBD-NAC causes selective necrosis to the pars recta of the proximal tubule , and is an organic anion it might be expected to be transported by the renal organic anion transport system .
	manualset3
263541	2	424197	15	NULL	NULL	NULL	NULL	selective necrosis 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because PCBD-NAC causes selective necrosis to the pars recta of the proximal tubule , and is an organic anion it might be expected to be transported by the renal organic anion transport system .
	manualset3
263542	3	424197	15	NULL	NULL	NULL	NULL	pars recta of the proximal tubule 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because PCBD-NAC causes selective necrosis to the pars recta of the proximal tubule , and is an organic anion it might be expected to be transported by the renal organic anion transport system .
	manualset3
263543	4	424197	15	NULL	NULL	NULL	NULL	organic anion	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because PCBD-NAC causes selective necrosis to the pars recta of the proximal tubule , and is an organic anion it might be expected to be transported by the renal organic anion transport system .
	manualset3
263544	5	424197	15	NULL	NULL	NULL	NULL	renal organic anion transport system	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because PCBD-NAC causes selective necrosis to the pars recta of the proximal tubule , and is an organic anion it might be expected to be transported by the renal organic anion transport system .
	manualset3
263545	1	424198	15	NULL	NULL	NULL	NULL	PNU145156E	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because PNU145156E inhibits tumor angiogenesis , it was selected for clinical development .
	manualset3
263546	2	424198	15	NULL	NULL	NULL	NULL	tumor angiogenesis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because PNU145156E inhibits tumor angiogenesis , it was selected for clinical development .
	manualset3
263547	3	424198	15	NULL	NULL	NULL	NULL	clinical development	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because PNU145156E inhibits tumor angiogenesis , it was selected for clinical development .
	manualset3
263548	1	424199	15	NULL	NULL	NULL	NULL	R5-like genotypes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because R5-like genotypes are more frequently associated with transmission , these observations suggest that the majority of women shedding HIV in genital secretions present a transmission risk .
	manualset3
263549	2	424199	15	NULL	NULL	NULL	NULL	transmission	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because R5-like genotypes are more frequently associated with transmission , these observations suggest that the majority of women shedding HIV in genital secretions present a transmission risk .
	manualset3
263550	3	424199	15	NULL	NULL	NULL	NULL	observations 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because R5-like genotypes are more frequently associated with transmission , these observations suggest that the majority of women shedding HIV in genital secretions present a transmission risk .
	manualset3
263551	4	424199	15	NULL	NULL	NULL	NULL	 women shedding HIV	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because R5-like genotypes are more frequently associated with transmission , these observations suggest that the majority of women shedding HIV in genital secretions present a transmission risk .
	manualset3
263552	5	424199	15	NULL	NULL	NULL	NULL	genital secretions	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because R5-like genotypes are more frequently associated with transmission , these observations suggest that the majority of women shedding HIV in genital secretions present a transmission risk .
	manualset3
263553	6	424199	15	NULL	NULL	NULL	NULL	transmission risk	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because R5-like genotypes are more frequently associated with transmission , these observations suggest that the majority of women shedding HIV in genital secretions present a transmission risk .
	manualset3
263554	1	424200	15	NULL	NULL	NULL	NULL	deletion of B cells 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because a PAH-induced , clonally nonrestricted deletion of B cells would have important implications for B cell repertoire development , the nature of the PAH-induced intracellular death signal was studied further .
	manualset3
263555	2	424200	15	NULL	NULL	NULL	NULL	implications	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because a PAH-induced , clonally nonrestricted deletion of B cells would have important implications for B cell repertoire development , the nature of the PAH-induced intracellular death signal was studied further .
	manualset3
263556	3	424200	15	NULL	NULL	NULL	NULL	B cell repertoire development	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because a PAH-induced , clonally nonrestricted deletion of B cells would have important implications for B cell repertoire development , the nature of the PAH-induced intracellular death signal was studied further .
	manualset3
263557	4	424200	15	NULL	NULL	NULL	NULL	nature 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because a PAH-induced , clonally nonrestricted deletion of B cells would have important implications for B cell repertoire development , the nature of the PAH-induced intracellular death signal was studied further .
	manualset3
263558	5	424200	15	NULL	NULL	NULL	NULL	PAH-induced intracellular death signal	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because a PAH-induced , clonally nonrestricted deletion of B cells would have important implications for B cell repertoire development , the nature of the PAH-induced intracellular death signal was studied further .
	manualset3
263562	1	424201	15	NULL	NULL	NULL	NULL	component of speaking	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because a major and very visible component of speaking a language is knowing how to create forms to carry messages , efforts to explain language production must confront long-standing questions about the relationship between structure and function in psychological explanation .
	manualset3
263563	2	424201	15	NULL	NULL	NULL	NULL	language 	Language												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because a major and very visible component of speaking a language is knowing how to create forms to carry messages , efforts to explain language production must confront long-standing questions about the relationship between structure and function in psychological explanation .
	manualset3
263564	3	424201	15	NULL	NULL	NULL	NULL	forms to carry messages	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because a major and very visible component of speaking a language is knowing how to create forms to carry messages , efforts to explain language production must confront long-standing questions about the relationship between structure and function in psychological explanation .
	manualset3
263565	4	424201	15	NULL	NULL	NULL	NULL	efforts	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because a major and very visible component of speaking a language is knowing how to create forms to carry messages , efforts to explain language production must confront long-standing questions about the relationship between structure and function in psychological explanation .
	manualset3
263566	5	424201	15	NULL	NULL	NULL	NULL	language production	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because a major and very visible component of speaking a language is knowing how to create forms to carry messages , efforts to explain language production must confront long-standing questions about the relationship between structure and function in psychological explanation .
	manualset3
263570	6	424201	15	NULL	NULL	NULL	NULL	long-standing questions	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because a major and very visible component of speaking a language is knowing how to create forms to carry messages , efforts to explain language production must confront long-standing questions about the relationship between structure and function in psychological explanation .
	manualset3
263571	7	424201	15	NULL	NULL	NULL	NULL	relationship	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because a major and very visible component of speaking a language is knowing how to create forms to carry messages , efforts to explain language production must confront long-standing questions about the relationship between structure and function in psychological explanation .
	manualset3
263572	8	424201	15	NULL	NULL	NULL	NULL	structure 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because a major and very visible component of speaking a language is knowing how to create forms to carry messages , efforts to explain language production must confront long-standing questions about the relationship between structure and function in psychological explanation .
	manualset3
263573	9	424201	15	NULL	NULL	NULL	NULL	function	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because a major and very visible component of speaking a language is knowing how to create forms to carry messages , efforts to explain language production must confront long-standing questions about the relationship between structure and function in psychological explanation .
	manualset3
263576	10	424201	15	NULL	NULL	NULL	NULL	psychological explanation 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because a major and very visible component of speaking a language is knowing how to create forms to carry messages , efforts to explain language production must confront long-standing questions about the relationship between structure and function in psychological explanation .
	manualset3
263580	1	424202	15	NULL	NULL	NULL	NULL	birds	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because all birds were killed as adults , results indicate the time of birth of neurons that survived to adulthood in different structures of the avian brain .
	manualset3
263581	2	424202	15	NULL	NULL	NULL	NULL	adults	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because all birds were killed as adults , results indicate the time of birth of neurons that survived to adulthood in different structures of the avian brain .
	manualset3
263582	3	424202	15	NULL	NULL	NULL	NULL	results	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because all birds were killed as adults , results indicate the time of birth of neurons that survived to adulthood in different structures of the avian brain .
	manualset3
263584	4	424202	15	NULL	NULL	NULL	NULL	time of birth 	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because all birds were killed as adults , results indicate the time of birth of neurons that survived to adulthood in different structures of the avian brain .
	manualset3
263586	5	424202	15	NULL	NULL	NULL	NULL	neurons	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because all birds were killed as adults , results indicate the time of birth of neurons that survived to adulthood in different structures of the avian brain .
	manualset3
263588	6	424202	15	NULL	NULL	NULL	NULL	adulthood	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because all birds were killed as adults , results indicate the time of birth of neurons that survived to adulthood in different structures of the avian brain .
	manualset3
263590	7	424202	15	NULL	NULL	NULL	NULL	structures	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because all birds were killed as adults , results indicate the time of birth of neurons that survived to adulthood in different structures of the avian brain .
	manualset3
263591	8	424202	15	NULL	NULL	NULL	NULL	avian brain	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because all birds were killed as adults , results indicate the time of birth of neurons that survived to adulthood in different structures of the avian brain .
	manualset3
263597	1	424203	15	NULL	NULL	NULL	NULL	androgen levels 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because androgen levels were in the physiological range , we conclude that the brain routinely enriches the estrogen content of blood in normal adult males of this species .
	manualset3
263600	2	424203	15	NULL	NULL	NULL	NULL	physiological range	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because androgen levels were in the physiological range , we conclude that the brain routinely enriches the estrogen content of blood in normal adult males of this species .
	manualset3
263601	3	424203	15	NULL	NULL	NULL	NULL	brain	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because androgen levels were in the physiological range , we conclude that the brain routinely enriches the estrogen content of blood in normal adult males of this species .
	manualset3
263603	4	424203	15	NULL	NULL	NULL	NULL	estrogen content of blood 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because androgen levels were in the physiological range , we conclude that the brain routinely enriches the estrogen content of blood in normal adult males of this species .
	manualset3
263606	5	424203	15	NULL	NULL	NULL	NULL	normal adult males	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because androgen levels were in the physiological range , we conclude that the brain routinely enriches the estrogen content of blood in normal adult males of this species .
	manualset3
263607	6	424203	15	NULL	NULL	NULL	NULL	 species 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because androgen levels were in the physiological range , we conclude that the brain routinely enriches the estrogen content of blood in normal adult males of this species .
	manualset3
263614	1	424204	15	NULL	NULL	NULL	NULL	polycythemia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because both polycythemia and increased eNOS expression are associated with chronic hypoxia-induced pulmonary hypertension , experiments were performed to test the hypothesis that increased hematocrit leads to upregulation of pulmonary eNOS and enhanced vascular production of NO independent of hypoxia .
	manualset3
263634	2	424204	15	NULL	NULL	NULL	NULL	increased eNOS expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because both polycythemia and increased eNOS expression are associated with chronic hypoxia-induced pulmonary hypertension , experiments were performed to test the hypothesis that increased hematocrit leads to upregulation of pulmonary eNOS and enhanced vascular production of NO independent of hypoxia .
	manualset3
263742	3	424204	15	NULL	NULL	NULL	NULL	chronic hypoxia-induced pulmonary hypertension	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because both polycythemia and increased eNOS expression are associated with chronic hypoxia-induced pulmonary hypertension , experiments were performed to test the hypothesis that increased hematocrit leads to upregulation of pulmonary eNOS and enhanced vascular production of NO independent of hypoxia .
	manualset3
263744	4	424204	15	NULL	NULL	NULL	NULL	experiments 	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because both polycythemia and increased eNOS expression are associated with chronic hypoxia-induced pulmonary hypertension , experiments were performed to test the hypothesis that increased hematocrit leads to upregulation of pulmonary eNOS and enhanced vascular production of NO independent of hypoxia .
	manualset3
263746	5	424204	15	NULL	NULL	NULL	NULL	hypothesis	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because both polycythemia and increased eNOS expression are associated with chronic hypoxia-induced pulmonary hypertension , experiments were performed to test the hypothesis that increased hematocrit leads to upregulation of pulmonary eNOS and enhanced vascular production of NO independent of hypoxia .
	manualset3
263749	6	424204	15	NULL	NULL	NULL	NULL	hematocrit 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because both polycythemia and increased eNOS expression are associated with chronic hypoxia-induced pulmonary hypertension , experiments were performed to test the hypothesis that increased hematocrit leads to upregulation of pulmonary eNOS and enhanced vascular production of NO independent of hypoxia .
	manualset3
263751	7	424204	15	NULL	NULL	NULL	NULL	upregulation 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because both polycythemia and increased eNOS expression are associated with chronic hypoxia-induced pulmonary hypertension , experiments were performed to test the hypothesis that increased hematocrit leads to upregulation of pulmonary eNOS and enhanced vascular production of NO independent of hypoxia .
	manualset3
263753	8	424204	15	NULL	NULL	NULL	NULL	pulmonary eNOS 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because both polycythemia and increased eNOS expression are associated with chronic hypoxia-induced pulmonary hypertension , experiments were performed to test the hypothesis that increased hematocrit leads to upregulation of pulmonary eNOS and enhanced vascular production of NO independent of hypoxia .
	manualset3
263754	9	424204	15	NULL	NULL	NULL	NULL	vascular production of NO	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because both polycythemia and increased eNOS expression are associated with chronic hypoxia-induced pulmonary hypertension , experiments were performed to test the hypothesis that increased hematocrit leads to upregulation of pulmonary eNOS and enhanced vascular production of NO independent of hypoxia .
	manualset3
263762	10	424204	15	NULL	NULL	NULL	NULL	hypoxia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because both polycythemia and increased eNOS expression are associated with chronic hypoxia-induced pulmonary hypertension , experiments were performed to test the hypothesis that increased hematocrit leads to upregulation of pulmonary eNOS and enhanced vascular production of NO independent of hypoxia .
	manualset3
263777	1	424205	15	NULL	NULL	NULL	NULL	bovUBE1L	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because bovUBE1L was purified through its interaction with rGST-ISG15 and shares significant amino acid and cDNA sequence identity with human UBE1L , it is concluded that it mediates conjugation of ISG15 to uterine proteins in response to the developing and attaching conceptus .
	manualset3
263780	2	424205	15	NULL	NULL	NULL	NULL	interaction	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because bovUBE1L was purified through its interaction with rGST-ISG15 and shares significant amino acid and cDNA sequence identity with human UBE1L , it is concluded that it mediates conjugation of ISG15 to uterine proteins in response to the developing and attaching conceptus .
	manualset3
263787	3	424205	15	NULL	NULL	NULL	NULL	rGST-ISG15	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because bovUBE1L was purified through its interaction with rGST-ISG15 and shares significant amino acid and cDNA sequence identity with human UBE1L , it is concluded that it mediates conjugation of ISG15 to uterine proteins in response to the developing and attaching conceptus .
	manualset3
263788	4	424205	15	NULL	NULL	NULL	NULL	amino acid	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because bovUBE1L was purified through its interaction with rGST-ISG15 and shares significant amino acid and cDNA sequence identity with human UBE1L , it is concluded that it mediates conjugation of ISG15 to uterine proteins in response to the developing and attaching conceptus .
	manualset3
263792	5	424205	15	NULL	NULL	NULL	NULL	cDNA sequence	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because bovUBE1L was purified through its interaction with rGST-ISG15 and shares significant amino acid and cDNA sequence identity with human UBE1L , it is concluded that it mediates conjugation of ISG15 to uterine proteins in response to the developing and attaching conceptus .
	manualset3
263794	6	424205	15	NULL	NULL	NULL	NULL	identity	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because bovUBE1L was purified through its interaction with rGST-ISG15 and shares significant amino acid and cDNA sequence identity with human UBE1L , it is concluded that it mediates conjugation of ISG15 to uterine proteins in response to the developing and attaching conceptus .
	manualset3
263798	7	424205	15	NULL	NULL	NULL	NULL	 human UBE1L	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because bovUBE1L was purified through its interaction with rGST-ISG15 and shares significant amino acid and cDNA sequence identity with human UBE1L , it is concluded that it mediates conjugation of ISG15 to uterine proteins in response to the developing and attaching conceptus .
	manualset3
263803	8	424205	15	NULL	NULL	NULL	NULL	ISG15	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because bovUBE1L was purified through its interaction with rGST-ISG15 and shares significant amino acid and cDNA sequence identity with human UBE1L , it is concluded that it mediates conjugation of ISG15 to uterine proteins in response to the developing and attaching conceptus .
	manualset3
263810	9	424205	15	NULL	NULL	NULL	NULL	uterine proteins 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because bovUBE1L was purified through its interaction with rGST-ISG15 and shares significant amino acid and cDNA sequence identity with human UBE1L , it is concluded that it mediates conjugation of ISG15 to uterine proteins in response to the developing and attaching conceptus .
	manualset3
263813	10	424205	15	NULL	NULL	NULL	NULL	response 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because bovUBE1L was purified through its interaction with rGST-ISG15 and shares significant amino acid and cDNA sequence identity with human UBE1L , it is concluded that it mediates conjugation of ISG15 to uterine proteins in response to the developing and attaching conceptus .
	manualset3
263820	11	424205	15	NULL	NULL	NULL	NULL	conceptus	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because bovUBE1L was purified through its interaction with rGST-ISG15 and shares significant amino acid and cDNA sequence identity with human UBE1L , it is concluded that it mediates conjugation of ISG15 to uterine proteins in response to the developing and attaching conceptus .
	manualset3
263827	1	424206	15	NULL	NULL	NULL	NULL	Experimental study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental study on the variations of the esophagogastric angle after Heller 's operation with & without left phrenico-exeresis ) .
	manualset3
263829	2	424206	15	NULL	NULL	NULL	NULL	variations	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental study on the variations of the esophagogastric angle after Heller 's operation with & without left phrenico-exeresis ) .
	manualset3
263831	3	424206	15	NULL	NULL	NULL	NULL	esophagogastric angle 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental study on the variations of the esophagogastric angle after Heller 's operation with & without left phrenico-exeresis ) .
	manualset3
263835	4	424206	15	NULL	NULL	NULL	NULL	Heller 's operation 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental study on the variations of the esophagogastric angle after Heller 's operation with & without left phrenico-exeresis ) .
	manualset3
263838	5	424206	15	NULL	NULL	NULL	NULL	phrenico-exeresis	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Experimental study on the variations of the esophagogastric angle after Heller 's operation with & without left phrenico-exeresis ) .
	manualset3
263839	1	424207	15	NULL	NULL	NULL	NULL	disruption	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because disruption of the actin cytoskeleton has been causally linked to steroidogenesis in various cell models , we sought to identify the cellular mechanisms that may modulate reorganization of the actin cytoskeleton and to determine whether cytoskeletal reorganization is required for steroidogenesis .
	manualset3
263841	2	424207	15	NULL	NULL	NULL	NULL	actin cytoskeleton	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because disruption of the actin cytoskeleton has been causally linked to steroidogenesis in various cell models , we sought to identify the cellular mechanisms that may modulate reorganization of the actin cytoskeleton and to determine whether cytoskeletal reorganization is required for steroidogenesis .
	manualset3
263895	3	424207	15	NULL	NULL	NULL	NULL	steroidogenesis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because disruption of the actin cytoskeleton has been causally linked to steroidogenesis in various cell models , we sought to identify the cellular mechanisms that may modulate reorganization of the actin cytoskeleton and to determine whether cytoskeletal reorganization is required for steroidogenesis .
	manualset3
263896	4	424207	15	NULL	NULL	NULL	NULL	 cell models	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because disruption of the actin cytoskeleton has been causally linked to steroidogenesis in various cell models , we sought to identify the cellular mechanisms that may modulate reorganization of the actin cytoskeleton and to determine whether cytoskeletal reorganization is required for steroidogenesis .
	manualset3
263897	5	424207	15	NULL	NULL	NULL	NULL	cellular mechanisms 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because disruption of the actin cytoskeleton has been causally linked to steroidogenesis in various cell models , we sought to identify the cellular mechanisms that may modulate reorganization of the actin cytoskeleton and to determine whether cytoskeletal reorganization is required for steroidogenesis .
	manualset3
263898	6	424207	15	NULL	NULL	NULL	NULL	reorganization of the actin cytoskeleton	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because disruption of the actin cytoskeleton has been causally linked to steroidogenesis in various cell models , we sought to identify the cellular mechanisms that may modulate reorganization of the actin cytoskeleton and to determine whether cytoskeletal reorganization is required for steroidogenesis .
	manualset3
263899	7	424207	15	NULL	NULL	NULL	NULL	cytoskeletal reorganization	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because disruption of the actin cytoskeleton has been causally linked to steroidogenesis in various cell models , we sought to identify the cellular mechanisms that may modulate reorganization of the actin cytoskeleton and to determine whether cytoskeletal reorganization is required for steroidogenesis .
	manualset3
263900	8	424207	15	NULL	NULL	NULL	NULL	steroidogenesis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because disruption of the actin cytoskeleton has been causally linked to steroidogenesis in various cell models , we sought to identify the cellular mechanisms that may modulate reorganization of the actin cytoskeleton and to determine whether cytoskeletal reorganization is required for steroidogenesis .
	manualset3
263901	1	424208	15	NULL	NULL	NULL	NULL	actin-based structures 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because distinct actin-based structures mediate diverse processes , many proteins are likely to make spatially and temporally regulated interactions with the Arp2/3 complex .
	manualset3
263902	2	424208	15	NULL	NULL	NULL	NULL	processes	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because distinct actin-based structures mediate diverse processes , many proteins are likely to make spatially and temporally regulated interactions with the Arp2/3 complex .
	manualset3
263903	3	424208	15	NULL	NULL	NULL	NULL	proteins	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because distinct actin-based structures mediate diverse processes , many proteins are likely to make spatially and temporally regulated interactions with the Arp2/3 complex .
	manualset3
263904	4	424208	15	NULL	NULL	NULL	NULL	spatially regulated interactions	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because distinct actin-based structures mediate diverse processes , many proteins are likely to make spatially and temporally regulated interactions with the Arp2/3 complex .
	manualset3
263905	5	424208	15	NULL	NULL	NULL	NULL	temporally regulated interactions 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because distinct actin-based structures mediate diverse processes , many proteins are likely to make spatially and temporally regulated interactions with the Arp2/3 complex .
	manualset3
263907	6	424208	15	NULL	NULL	NULL	NULL	Arp2/3 complex	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because distinct actin-based structures mediate diverse processes , many proteins are likely to make spatially and temporally regulated interactions with the Arp2/3 complex .
	manualset3
263911	1	424209	15	NULL	NULL	NULL	NULL	oocyte	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because each oocyte is capable of recombining nanogram quantities of linear DNA , this system offers exceptional opportunities for detailed molecular analysis of the recombination process in a higher organism .
	manualset3
263912	2	424209	15	NULL	NULL	NULL	NULL	recombining	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because each oocyte is capable of recombining nanogram quantities of linear DNA , this system offers exceptional opportunities for detailed molecular analysis of the recombination process in a higher organism .
	manualset3
263913	3	424209	15	NULL	NULL	NULL	NULL	nanogram quantities	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because each oocyte is capable of recombining nanogram quantities of linear DNA , this system offers exceptional opportunities for detailed molecular analysis of the recombination process in a higher organism .
	manualset3
263914	4	424209	15	NULL	NULL	NULL	NULL	linear DNA	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because each oocyte is capable of recombining nanogram quantities of linear DNA , this system offers exceptional opportunities for detailed molecular analysis of the recombination process in a higher organism .
	manualset3
263916	5	424209	15	NULL	NULL	NULL	NULL	system	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because each oocyte is capable of recombining nanogram quantities of linear DNA , this system offers exceptional opportunities for detailed molecular analysis of the recombination process in a higher organism .
	manualset3
263919	6	424209	15	NULL	NULL	NULL	NULL	opportunities 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because each oocyte is capable of recombining nanogram quantities of linear DNA , this system offers exceptional opportunities for detailed molecular analysis of the recombination process in a higher organism .
	manualset3
263921	7	424209	15	NULL	NULL	NULL	NULL	molecular analysis 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because each oocyte is capable of recombining nanogram quantities of linear DNA , this system offers exceptional opportunities for detailed molecular analysis of the recombination process in a higher organism .
	manualset3
263923	8	424209	15	NULL	NULL	NULL	NULL	recombination process	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because each oocyte is capable of recombining nanogram quantities of linear DNA , this system offers exceptional opportunities for detailed molecular analysis of the recombination process in a higher organism .
	manualset3
263925	9	424209	15	NULL	NULL	NULL	NULL	 organism 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because each oocyte is capable of recombining nanogram quantities of linear DNA , this system offers exceptional opportunities for detailed molecular analysis of the recombination process in a higher organism .
	manualset3
263927	1	424210	15	NULL	NULL	NULL	NULL	ejection fraction	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because ejection fraction and pulmonary capillary wedge pressure were not significantly changed even after the 20 mg dose , bisoprolol has only mild negative inotropic effects and seems hemodynamically safe .
	manualset3
263929	2	424210	15	NULL	NULL	NULL	NULL	pulmonary capillary wedge pressure 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because ejection fraction and pulmonary capillary wedge pressure were not significantly changed even after the 20 mg dose , bisoprolol has only mild negative inotropic effects and seems hemodynamically safe .
	manualset3
263932	3	424210	15	NULL	NULL	NULL	NULL	20 mg dose 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because ejection fraction and pulmonary capillary wedge pressure were not significantly changed even after the 20 mg dose , bisoprolol has only mild negative inotropic effects and seems hemodynamically safe .
	manualset3
263933	4	424210	15	NULL	NULL	NULL	NULL	bisoprolol	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because ejection fraction and pulmonary capillary wedge pressure were not significantly changed even after the 20 mg dose , bisoprolol has only mild negative inotropic effects and seems hemodynamically safe .
	manualset3
263936	5	424210	15	NULL	NULL	NULL	NULL	inotropic effects 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because ejection fraction and pulmonary capillary wedge pressure were not significantly changed even after the 20 mg dose , bisoprolol has only mild negative inotropic effects and seems hemodynamically safe .
	manualset3
263938	1	424211	15	NULL	NULL	NULL	NULL	epidemiologic studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because epidemiologic studies are often used to evaluate modest differences in risk factors , it is essential to minimize sources of errors and to maximize sensitivity , reproducibility , and specificity .
	manualset3
263939	2	424211	15	NULL	NULL	NULL	NULL	differences	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because epidemiologic studies are often used to evaluate modest differences in risk factors , it is essential to minimize sources of errors and to maximize sensitivity , reproducibility , and specificity .
	manualset3
263940	3	424211	15	NULL	NULL	NULL	NULL	risk factors	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because epidemiologic studies are often used to evaluate modest differences in risk factors , it is essential to minimize sources of errors and to maximize sensitivity , reproducibility , and specificity .
	manualset3
263941	4	424211	15	NULL	NULL	NULL	NULL	sources of errors	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because epidemiologic studies are often used to evaluate modest differences in risk factors , it is essential to minimize sources of errors and to maximize sensitivity , reproducibility , and specificity .
	manualset3
263942	5	424211	15	NULL	NULL	NULL	NULL	sensitivity 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because epidemiologic studies are often used to evaluate modest differences in risk factors , it is essential to minimize sources of errors and to maximize sensitivity , reproducibility , and specificity .
	manualset3
263943	6	424211	15	NULL	NULL	NULL	NULL	reproducibility	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because epidemiologic studies are often used to evaluate modest differences in risk factors , it is essential to minimize sources of errors and to maximize sensitivity , reproducibility , and specificity .
	manualset3
263944	7	424211	15	NULL	NULL	NULL	NULL	specificity	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because epidemiologic studies are often used to evaluate modest differences in risk factors , it is essential to minimize sources of errors and to maximize sensitivity , reproducibility , and specificity .
	manualset3
263947	1	424212	15	NULL	NULL	NULL	NULL	ethanol	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because ethanol ingestion lowers delta-aminolevulinic acid dehydratase ( ALAD ) activity in liver and red cells , effects of ethanol and acetaldehyde on ALAD in rat liver cytosol were studied .
	manualset3
263949	2	424212	15	NULL	NULL	NULL	NULL	ingestion 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because ethanol ingestion lowers delta-aminolevulinic acid dehydratase ( ALAD ) activity in liver and red cells , effects of ethanol and acetaldehyde on ALAD in rat liver cytosol were studied .
	manualset3
263952	3	424212	15	NULL	NULL	NULL	NULL	delta-aminolevulinic acid dehydratase ( ALAD ) activity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because ethanol ingestion lowers delta-aminolevulinic acid dehydratase ( ALAD ) activity in liver and red cells , effects of ethanol and acetaldehyde on ALAD in rat liver cytosol were studied .
	manualset3
263954	4	424212	15	NULL	NULL	NULL	NULL	liver	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because ethanol ingestion lowers delta-aminolevulinic acid dehydratase ( ALAD ) activity in liver and red cells , effects of ethanol and acetaldehyde on ALAD in rat liver cytosol were studied .
	manualset3
263955	5	424212	15	NULL	NULL	NULL	NULL	red cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because ethanol ingestion lowers delta-aminolevulinic acid dehydratase ( ALAD ) activity in liver and red cells , effects of ethanol and acetaldehyde on ALAD in rat liver cytosol were studied .
	manualset3
263958	6	424212	15	NULL	NULL	NULL	NULL	effects	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because ethanol ingestion lowers delta-aminolevulinic acid dehydratase ( ALAD ) activity in liver and red cells , effects of ethanol and acetaldehyde on ALAD in rat liver cytosol were studied .
	manualset3
263960	7	424212	15	NULL	NULL	NULL	NULL	ethanol 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because ethanol ingestion lowers delta-aminolevulinic acid dehydratase ( ALAD ) activity in liver and red cells , effects of ethanol and acetaldehyde on ALAD in rat liver cytosol were studied .
	manualset3
263961	8	424212	15	NULL	NULL	NULL	NULL	acetaldehyde	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because ethanol ingestion lowers delta-aminolevulinic acid dehydratase ( ALAD ) activity in liver and red cells , effects of ethanol and acetaldehyde on ALAD in rat liver cytosol were studied .
	manualset3
263963	9	424212	15	NULL	NULL	NULL	NULL	ALAD	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because ethanol ingestion lowers delta-aminolevulinic acid dehydratase ( ALAD ) activity in liver and red cells , effects of ethanol and acetaldehyde on ALAD in rat liver cytosol were studied .
	manualset3
263965	10	424212	15	NULL	NULL	NULL	NULL	rat liver cytosol 	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because ethanol ingestion lowers delta-aminolevulinic acid dehydratase ( ALAD ) activity in liver and red cells , effects of ethanol and acetaldehyde on ALAD in rat liver cytosol were studied .
	manualset3
263983	1	424213	15	NULL	NULL	NULL	NULL	gangliogliomas	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because gangliogliomas usually have a good prognosis following resection , it is important to clearly distinguish them from other NF1-associated lesions , even though ganglioglioma of the thoracolumbar spinal cord , including the conus medullaris , is an extremely rare condition .
	manualset3
263984	2	424213	15	NULL	NULL	NULL	NULL	prognosis	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because gangliogliomas usually have a good prognosis following resection , it is important to clearly distinguish them from other NF1-associated lesions , even though ganglioglioma of the thoracolumbar spinal cord , including the conus medullaris , is an extremely rare condition .
	manualset3
263985	3	424213	15	NULL	NULL	NULL	NULL	resection 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because gangliogliomas usually have a good prognosis following resection , it is important to clearly distinguish them from other NF1-associated lesions , even though ganglioglioma of the thoracolumbar spinal cord , including the conus medullaris , is an extremely rare condition .
	manualset3
263986	4	424213	15	NULL	NULL	NULL	NULL	NF1-associated lesions 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because gangliogliomas usually have a good prognosis following resection , it is important to clearly distinguish them from other NF1-associated lesions , even though ganglioglioma of the thoracolumbar spinal cord , including the conus medullaris , is an extremely rare condition .
	manualset3
263987	5	424213	15	NULL	NULL	NULL	NULL	ganglioglioma	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because gangliogliomas usually have a good prognosis following resection , it is important to clearly distinguish them from other NF1-associated lesions , even though ganglioglioma of the thoracolumbar spinal cord , including the conus medullaris , is an extremely rare condition .
	manualset3
263988	6	424213	15	NULL	NULL	NULL	NULL	thoracolumbar spinal cord	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because gangliogliomas usually have a good prognosis following resection , it is important to clearly distinguish them from other NF1-associated lesions , even though ganglioglioma of the thoracolumbar spinal cord , including the conus medullaris , is an extremely rare condition .
	manualset3
263989	7	424213	15	NULL	NULL	NULL	NULL	conus medullaris	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because gangliogliomas usually have a good prognosis following resection , it is important to clearly distinguish them from other NF1-associated lesions , even though ganglioglioma of the thoracolumbar spinal cord , including the conus medullaris , is an extremely rare condition .
	manualset3
263990	8	424213	15	NULL	NULL	NULL	NULL	rare condition	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because gangliogliomas usually have a good prognosis following resection , it is important to clearly distinguish them from other NF1-associated lesions , even though ganglioglioma of the thoracolumbar spinal cord , including the conus medullaris , is an extremely rare condition .
	manualset3
263991	1	424214	15	NULL	NULL	NULL	NULL	gastric carcinoma 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because gastric carcinoma associated with bilateral chylothorax is very rare , we report the results of our study with some discussion based on a review of the literature .
	manualset3
263992	2	424214	15	NULL	NULL	NULL	NULL	bilateral chylothorax	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because gastric carcinoma associated with bilateral chylothorax is very rare , we report the results of our study with some discussion based on a review of the literature .
	manualset3
263993	3	424214	15	NULL	NULL	NULL	NULL	results	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because gastric carcinoma associated with bilateral chylothorax is very rare , we report the results of our study with some discussion based on a review of the literature .
	manualset3
263994	4	424214	15	NULL	NULL	NULL	NULL	study 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because gastric carcinoma associated with bilateral chylothorax is very rare , we report the results of our study with some discussion based on a review of the literature .
	manualset3
263995	5	424214	15	NULL	NULL	NULL	NULL	discussion	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because gastric carcinoma associated with bilateral chylothorax is very rare , we report the results of our study with some discussion based on a review of the literature .
	manualset3
263996	6	424214	15	NULL	NULL	NULL	NULL	review of the literature 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because gastric carcinoma associated with bilateral chylothorax is very rare , we report the results of our study with some discussion based on a review of the literature .
	manualset3
263997	1	424215	15	NULL	NULL	NULL	NULL	initial neuroprotection	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because initial neuroprotection is sometimes transient and may not subserve functional recovery , especially on demanding tasks , the authors examined whether postischemic cooling would persistently reduce infarction and forelimb reaching deficits after MCAO .
	manualset3
263998	2	424215	15	NULL	NULL	NULL	NULL	functional recovery	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because initial neuroprotection is sometimes transient and may not subserve functional recovery , especially on demanding tasks , the authors examined whether postischemic cooling would persistently reduce infarction and forelimb reaching deficits after MCAO .
	manualset3
263999	3	424215	15	NULL	NULL	NULL	NULL	tasks	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because initial neuroprotection is sometimes transient and may not subserve functional recovery , especially on demanding tasks , the authors examined whether postischemic cooling would persistently reduce infarction and forelimb reaching deficits after MCAO .
	manualset3
264000	4	424215	15	NULL	NULL	NULL	NULL	authors	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because initial neuroprotection is sometimes transient and may not subserve functional recovery , especially on demanding tasks , the authors examined whether postischemic cooling would persistently reduce infarction and forelimb reaching deficits after MCAO .
	manualset3
264001	5	424215	15	NULL	NULL	NULL	NULL	postischemic cooling 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because initial neuroprotection is sometimes transient and may not subserve functional recovery , especially on demanding tasks , the authors examined whether postischemic cooling would persistently reduce infarction and forelimb reaching deficits after MCAO .
	manualset3
264002	6	424215	15	NULL	NULL	NULL	NULL	infarction 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because initial neuroprotection is sometimes transient and may not subserve functional recovery , especially on demanding tasks , the authors examined whether postischemic cooling would persistently reduce infarction and forelimb reaching deficits after MCAO .
	manualset3
264003	7	424215	15	NULL	NULL	NULL	NULL	forelimb reaching deficits 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because initial neuroprotection is sometimes transient and may not subserve functional recovery , especially on demanding tasks , the authors examined whether postischemic cooling would persistently reduce infarction and forelimb reaching deficits after MCAO .
	manualset3
264004	8	424215	15	NULL	NULL	NULL	NULL	MCAO	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because initial neuroprotection is sometimes transient and may not subserve functional recovery , especially on demanding tasks , the authors examined whether postischemic cooling would persistently reduce infarction and forelimb reaching deficits after MCAO .
	manualset3
264005	1	424216	15	NULL	NULL	NULL	NULL	vanilloid	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because it is possible to examine vanilloid and heat sensitivities in vitro and in vivo , X. tropicalis could be the ideal experimental lower vertebrate animal for the study of TRPV1 function .
	manualset3
264006	2	424216	15	NULL	NULL	NULL	NULL	heat sensitivities	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because it is possible to examine vanilloid and heat sensitivities in vitro and in vivo , X. tropicalis could be the ideal experimental lower vertebrate animal for the study of TRPV1 function .
	manualset3
264007	3	424216	15	NULL	NULL	NULL	NULL	X. tropicalis 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because it is possible to examine vanilloid and heat sensitivities in vitro and in vivo , X. tropicalis could be the ideal experimental lower vertebrate animal for the study of TRPV1 function .
	manualset3
264008	4	424216	15	NULL	NULL	NULL	NULL	experimental lower vertebrate animal	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because it is possible to examine vanilloid and heat sensitivities in vitro and in vivo , X. tropicalis could be the ideal experimental lower vertebrate animal for the study of TRPV1 function .
	manualset3
264009	5	424216	15	NULL	NULL	NULL	NULL	study of TRPV1 function	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because it is possible to examine vanilloid and heat sensitivities in vitro and in vivo , X. tropicalis could be the ideal experimental lower vertebrate animal for the study of TRPV1 function .
	manualset3
264010	1	424217	15	NULL	NULL	NULL	NULL	minichromosome maintenance complex proteins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because minichromosome maintenance complex proteins are thought to function as a heterohexamer , loading of Mcm2 - , Mcm4 - , and Mcm7-depleted complexes is likely to underlie the S phase defects observed in cyclin E-deregulated cells , consistent with a role for minichromosome maintenance complex proteins in initiation of replication and fork movement .
	manualset3
264011	2	424217	15	NULL	NULL	NULL	NULL	heterohexamer	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because minichromosome maintenance complex proteins are thought to function as a heterohexamer , loading of Mcm2 - , Mcm4 - , and Mcm7-depleted complexes is likely to underlie the S phase defects observed in cyclin E-deregulated cells , consistent with a role for minichromosome maintenance complex proteins in initiation of replication and fork movement .
	manualset3
264012	3	424217	15	NULL	NULL	NULL	NULL	Mcm2 - depleted complexes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because minichromosome maintenance complex proteins are thought to function as a heterohexamer , loading of Mcm2 - , Mcm4 - , and Mcm7-depleted complexes is likely to underlie the S phase defects observed in cyclin E-deregulated cells , consistent with a role for minichromosome maintenance complex proteins in initiation of replication and fork movement .
	manualset3
264013	4	424217	15	NULL	NULL	NULL	NULL	Mcm4 -depleted complexes 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because minichromosome maintenance complex proteins are thought to function as a heterohexamer , loading of Mcm2 - , Mcm4 - , and Mcm7-depleted complexes is likely to underlie the S phase defects observed in cyclin E-deregulated cells , consistent with a role for minichromosome maintenance complex proteins in initiation of replication and fork movement .
	manualset3
264014	5	424217	15	NULL	NULL	NULL	NULL	Mcm7-depleted complexes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because minichromosome maintenance complex proteins are thought to function as a heterohexamer , loading of Mcm2 - , Mcm4 - , and Mcm7-depleted complexes is likely to underlie the S phase defects observed in cyclin E-deregulated cells , consistent with a role for minichromosome maintenance complex proteins in initiation of replication and fork movement .
	manualset3
264015	6	424217	15	NULL	NULL	NULL	NULL	S phase defects	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because minichromosome maintenance complex proteins are thought to function as a heterohexamer , loading of Mcm2 - , Mcm4 - , and Mcm7-depleted complexes is likely to underlie the S phase defects observed in cyclin E-deregulated cells , consistent with a role for minichromosome maintenance complex proteins in initiation of replication and fork movement .
	manualset3
264016	7	424217	15	NULL	NULL	NULL	NULL	cyclin E-deregulated cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because minichromosome maintenance complex proteins are thought to function as a heterohexamer , loading of Mcm2 - , Mcm4 - , and Mcm7-depleted complexes is likely to underlie the S phase defects observed in cyclin E-deregulated cells , consistent with a role for minichromosome maintenance complex proteins in initiation of replication and fork movement .
	manualset3
264017	8	424217	15	NULL	NULL	NULL	NULL	role	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because minichromosome maintenance complex proteins are thought to function as a heterohexamer , loading of Mcm2 - , Mcm4 - , and Mcm7-depleted complexes is likely to underlie the S phase defects observed in cyclin E-deregulated cells , consistent with a role for minichromosome maintenance complex proteins in initiation of replication and fork movement .
	manualset3
264018	9	424217	15	NULL	NULL	NULL	NULL	minichromosome maintenance complex proteins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because minichromosome maintenance complex proteins are thought to function as a heterohexamer , loading of Mcm2 - , Mcm4 - , and Mcm7-depleted complexes is likely to underlie the S phase defects observed in cyclin E-deregulated cells , consistent with a role for minichromosome maintenance complex proteins in initiation of replication and fork movement .
	manualset3
264019	10	424217	15	NULL	NULL	NULL	NULL	initiation of replication	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because minichromosome maintenance complex proteins are thought to function as a heterohexamer , loading of Mcm2 - , Mcm4 - , and Mcm7-depleted complexes is likely to underlie the S phase defects observed in cyclin E-deregulated cells , consistent with a role for minichromosome maintenance complex proteins in initiation of replication and fork movement .
	manualset3
264020	11	424217	15	NULL	NULL	NULL	NULL	fork movement	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because minichromosome maintenance complex proteins are thought to function as a heterohexamer , loading of Mcm2 - , Mcm4 - , and Mcm7-depleted complexes is likely to underlie the S phase defects observed in cyclin E-deregulated cells , consistent with a role for minichromosome maintenance complex proteins in initiation of replication and fork movement .
	manualset3
264021	1	424218	15	NULL	NULL	NULL	NULL	emphasis	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of an increased emphasis on beauty and health , cosmetic dentistry has been the thrust to the forefront of many practices .
	manualset3
264022	2	424218	15	NULL	NULL	NULL	NULL	beauty	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of an increased emphasis on beauty and health , cosmetic dentistry has been the thrust to the forefront of many practices .
	manualset3
264023	3	424218	15	NULL	NULL	NULL	NULL	health 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of an increased emphasis on beauty and health , cosmetic dentistry has been the thrust to the forefront of many practices .
	manualset3
264024	4	424218	15	NULL	NULL	NULL	NULL	cosmetic dentistry 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of an increased emphasis on beauty and health , cosmetic dentistry has been the thrust to the forefront of many practices .
	manualset3
264025	5	424218	15	NULL	NULL	NULL	NULL	thrust	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of an increased emphasis on beauty and health , cosmetic dentistry has been the thrust to the forefront of many practices .
	manualset3
264026	6	424218	15	NULL	NULL	NULL	NULL	forefront	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of an increased emphasis on beauty and health , cosmetic dentistry has been the thrust to the forefront of many practices .
	manualset3
264027	7	424218	15	NULL	NULL	NULL	NULL	practices	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of an increased emphasis on beauty and health , cosmetic dentistry has been the thrust to the forefront of many practices .
	manualset3
264028	1	424219	15	NULL	NULL	NULL	NULL	Expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Expression , purification and application of bla ( TEM-116 ) extended-spectrum beta-lactamase ) .
	manualset3
264029	2	424219	15	NULL	NULL	NULL	NULL	purification	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Expression , purification and application of bla ( TEM-116 ) extended-spectrum beta-lactamase ) .
	manualset3
264030	3	424219	15	NULL	NULL	NULL	NULL	application	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Expression , purification and application of bla ( TEM-116 ) extended-spectrum beta-lactamase ) .
	manualset3
264031	4	424219	15	NULL	NULL	NULL	NULL	bla ( TEM-116 ) extended-spectrum beta-lactamase 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Expression , purification and application of bla ( TEM-116 ) extended-spectrum beta-lactamase ) .
	manualset3
264032	1	424220	15	NULL	NULL	NULL	NULL	modifications	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of many modifications that can be applied to chitosan , e.g. combining with drugs , growth factors , nerve stem cells , and connecting with other biopolymers , this material seems very promising .
	manualset3
264033	2	424220	15	NULL	NULL	NULL	NULL	chitosan	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of many modifications that can be applied to chitosan , e.g. combining with drugs , growth factors , nerve stem cells , and connecting with other biopolymers , this material seems very promising .
	manualset3
264034	3	424220	15	NULL	NULL	NULL	NULL	combining with drugs	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of many modifications that can be applied to chitosan , e.g. combining with drugs , growth factors , nerve stem cells , and connecting with other biopolymers , this material seems very promising .
	manualset3
264035	4	424220	15	NULL	NULL	NULL	NULL	growth factors	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of many modifications that can be applied to chitosan , e.g. combining with drugs , growth factors , nerve stem cells , and connecting with other biopolymers , this material seems very promising .
	manualset3
264036	5	424220	15	NULL	NULL	NULL	NULL	nerve stem cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of many modifications that can be applied to chitosan , e.g. combining with drugs , growth factors , nerve stem cells , and connecting with other biopolymers , this material seems very promising .
	manualset3
264037	6	424220	15	NULL	NULL	NULL	NULL	biopolymers	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of many modifications that can be applied to chitosan , e.g. combining with drugs , growth factors , nerve stem cells , and connecting with other biopolymers , this material seems very promising .
	manualset3
264038	7	424220	15	NULL	NULL	NULL	NULL	material	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of many modifications that can be applied to chitosan , e.g. combining with drugs , growth factors , nerve stem cells , and connecting with other biopolymers , this material seems very promising .
	manualset3
264255	1	424221	15	NULL	NULL	NULL	NULL	similarities	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of similarities in the pathophysiology of multiple myeloma and Waldenstrom 's macroglobulinemia ( WM ) , we investigated DNA samples from 20 bone marrow biopsies with WM for the detection of KSHV by PCR ( KS330/ORF26 ) .
	manualset3
264256	2	424221	15	NULL	NULL	NULL	NULL	pathophysiology	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of similarities in the pathophysiology of multiple myeloma and Waldenstrom 's macroglobulinemia ( WM ) , we investigated DNA samples from 20 bone marrow biopsies with WM for the detection of KSHV by PCR ( KS330/ORF26 ) .
	manualset3
264269	3	424221	15	NULL	NULL	NULL	NULL	multiple myeloma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of similarities in the pathophysiology of multiple myeloma and Waldenstrom 's macroglobulinemia ( WM ) , we investigated DNA samples from 20 bone marrow biopsies with WM for the detection of KSHV by PCR ( KS330/ORF26 ) .
	manualset3
264271	4	424221	15	NULL	NULL	NULL	NULL	Waldenstrom 's macroglobulinemia ( WM )	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of similarities in the pathophysiology of multiple myeloma and Waldenstrom 's macroglobulinemia ( WM ) , we investigated DNA samples from 20 bone marrow biopsies with WM for the detection of KSHV by PCR ( KS330/ORF26 ) .
	manualset3
264273	5	424221	15	NULL	NULL	NULL	NULL	DNA samples	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of similarities in the pathophysiology of multiple myeloma and Waldenstrom 's macroglobulinemia ( WM ) , we investigated DNA samples from 20 bone marrow biopsies with WM for the detection of KSHV by PCR ( KS330/ORF26 ) .
	manualset3
264274	6	424221	15	NULL	NULL	NULL	NULL	20	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of similarities in the pathophysiology of multiple myeloma and Waldenstrom 's macroglobulinemia ( WM ) , we investigated DNA samples from 20 bone marrow biopsies with WM for the detection of KSHV by PCR ( KS330/ORF26 ) .
	manualset3
264276	7	424221	15	NULL	NULL	NULL	NULL	bone marrow biopsies	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of similarities in the pathophysiology of multiple myeloma and Waldenstrom 's macroglobulinemia ( WM ) , we investigated DNA samples from 20 bone marrow biopsies with WM for the detection of KSHV by PCR ( KS330/ORF26 ) .
	manualset3
264277	8	424221	15	NULL	NULL	NULL	NULL	WM	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of similarities in the pathophysiology of multiple myeloma and Waldenstrom 's macroglobulinemia ( WM ) , we investigated DNA samples from 20 bone marrow biopsies with WM for the detection of KSHV by PCR ( KS330/ORF26 ) .
	manualset3
264279	9	424221	15	NULL	NULL	NULL	NULL	detection	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of similarities in the pathophysiology of multiple myeloma and Waldenstrom 's macroglobulinemia ( WM ) , we investigated DNA samples from 20 bone marrow biopsies with WM for the detection of KSHV by PCR ( KS330/ORF26 ) .
	manualset3
264282	10	424221	15	NULL	NULL	NULL	NULL	KSHV	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of similarities in the pathophysiology of multiple myeloma and Waldenstrom 's macroglobulinemia ( WM ) , we investigated DNA samples from 20 bone marrow biopsies with WM for the detection of KSHV by PCR ( KS330/ORF26 ) .
	manualset3
264283	11	424221	15	NULL	NULL	NULL	NULL	PCR ( KS330/ORF26 )	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of similarities in the pathophysiology of multiple myeloma and Waldenstrom 's macroglobulinemia ( WM ) , we investigated DNA samples from 20 bone marrow biopsies with WM for the detection of KSHV by PCR ( KS330/ORF26 ) .
	manualset3
264287	1	424222	15	NULL	NULL	NULL	NULL	proximity	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the close proximity to the brain stem , the tumor could not be removed completely .
	manualset3
264288	2	424222	15	NULL	NULL	NULL	NULL	brain stem	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the close proximity to the brain stem , the tumor could not be removed completely .
	manualset3
264289	3	424222	15	NULL	NULL	NULL	NULL	tumor 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the close proximity to the brain stem , the tumor could not be removed completely .
	manualset3
264290	1	424223	15	NULL	NULL	NULL	NULL	difference	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the difference in bacterial invasiveness , we may need to choose a suitable cell system for each target pathogen .
	manualset3
264291	2	424223	15	NULL	NULL	NULL	NULL	bacterial invasiveness	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the difference in bacterial invasiveness , we may need to choose a suitable cell system for each target pathogen .
	manualset3
264292	3	424223	15	NULL	NULL	NULL	NULL	cell system	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the difference in bacterial invasiveness , we may need to choose a suitable cell system for each target pathogen .
	manualset3
264316	4	424223	15	NULL	NULL	NULL	NULL	target pathogen	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the difference in bacterial invasiveness , we may need to choose a suitable cell system for each target pathogen .
	manualset3
264317	1	424224	15	NULL	NULL	NULL	NULL	results 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the encouraging results even in patients older than 60 years , hemopoietic stem cell grafting should be seriously considered as part of an overall treatment strategy , in order to avoid irreversible normal hemopoietic stem cell damage from nitrosoureas and radiation to marrow-containing bones .
	manualset3
264318	2	424224	15	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the encouraging results even in patients older than 60 years , hemopoietic stem cell grafting should be seriously considered as part of an overall treatment strategy , in order to avoid irreversible normal hemopoietic stem cell damage from nitrosoureas and radiation to marrow-containing bones .
	manualset3
264319	3	424224	15	NULL	NULL	NULL	NULL	60 years	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the encouraging results even in patients older than 60 years , hemopoietic stem cell grafting should be seriously considered as part of an overall treatment strategy , in order to avoid irreversible normal hemopoietic stem cell damage from nitrosoureas and radiation to marrow-containing bones .
	manualset3
264320	4	424224	15	NULL	NULL	NULL	NULL	hemopoietic stem cell grafting	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the encouraging results even in patients older than 60 years , hemopoietic stem cell grafting should be seriously considered as part of an overall treatment strategy , in order to avoid irreversible normal hemopoietic stem cell damage from nitrosoureas and radiation to marrow-containing bones .
	manualset3
264321	5	424224	15	NULL	NULL	NULL	NULL	overall treatment strategy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the encouraging results even in patients older than 60 years , hemopoietic stem cell grafting should be seriously considered as part of an overall treatment strategy , in order to avoid irreversible normal hemopoietic stem cell damage from nitrosoureas and radiation to marrow-containing bones .
	manualset3
264322	6	424224	15	NULL	NULL	NULL	NULL	hemopoietic stem cell damage 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the encouraging results even in patients older than 60 years , hemopoietic stem cell grafting should be seriously considered as part of an overall treatment strategy , in order to avoid irreversible normal hemopoietic stem cell damage from nitrosoureas and radiation to marrow-containing bones .
	manualset3
264323	7	424224	15	NULL	NULL	NULL	NULL	nitrosoureas 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the encouraging results even in patients older than 60 years , hemopoietic stem cell grafting should be seriously considered as part of an overall treatment strategy , in order to avoid irreversible normal hemopoietic stem cell damage from nitrosoureas and radiation to marrow-containing bones .
	manualset3
264324	8	424224	15	NULL	NULL	NULL	NULL	radiation 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the encouraging results even in patients older than 60 years , hemopoietic stem cell grafting should be seriously considered as part of an overall treatment strategy , in order to avoid irreversible normal hemopoietic stem cell damage from nitrosoureas and radiation to marrow-containing bones .
	manualset3
264325	9	424224	15	NULL	NULL	NULL	NULL	marrow-containing bones	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the encouraging results even in patients older than 60 years , hemopoietic stem cell grafting should be seriously considered as part of an overall treatment strategy , in order to avoid irreversible normal hemopoietic stem cell damage from nitrosoureas and radiation to marrow-containing bones .
	manualset3
264326	1	424225	15	NULL	NULL	NULL	NULL	heterogeneity 	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the heterogeneity of the biological behavior of desmoids , including long periods of stable disease or even spontaneous regression , treatment needs to be individualized to optimize local tumor control and preserve patients ' quality of life .
	manualset3
264327	2	424225	15	NULL	NULL	NULL	NULL	biological behavior of desmoids	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the heterogeneity of the biological behavior of desmoids , including long periods of stable disease or even spontaneous regression , treatment needs to be individualized to optimize local tumor control and preserve patients ' quality of life .
	manualset3
264328	3	424225	15	NULL	NULL	NULL	NULL	long periods	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the heterogeneity of the biological behavior of desmoids , including long periods of stable disease or even spontaneous regression , treatment needs to be individualized to optimize local tumor control and preserve patients ' quality of life .
	manualset3
264329	4	424225	15	NULL	NULL	NULL	NULL	stable disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the heterogeneity of the biological behavior of desmoids , including long periods of stable disease or even spontaneous regression , treatment needs to be individualized to optimize local tumor control and preserve patients ' quality of life .
	manualset3
264330	5	424225	15	NULL	NULL	NULL	NULL	spontaneous regression	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the heterogeneity of the biological behavior of desmoids , including long periods of stable disease or even spontaneous regression , treatment needs to be individualized to optimize local tumor control and preserve patients ' quality of life .
	manualset3
264331	6	424225	15	NULL	NULL	NULL	NULL	 treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the heterogeneity of the biological behavior of desmoids , including long periods of stable disease or even spontaneous regression , treatment needs to be individualized to optimize local tumor control and preserve patients ' quality of life .
	manualset3
264332	7	424225	15	NULL	NULL	NULL	NULL	local tumor control 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the heterogeneity of the biological behavior of desmoids , including long periods of stable disease or even spontaneous regression , treatment needs to be individualized to optimize local tumor control and preserve patients ' quality of life .
	manualset3
264333	8	424225	15	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the heterogeneity of the biological behavior of desmoids , including long periods of stable disease or even spontaneous regression , treatment needs to be individualized to optimize local tumor control and preserve patients ' quality of life .
	manualset3
264334	9	424225	15	NULL	NULL	NULL	NULL	quality of life	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the heterogeneity of the biological behavior of desmoids , including long periods of stable disease or even spontaneous regression , treatment needs to be individualized to optimize local tumor control and preserve patients ' quality of life .
	manualset3
264336	1	424226	15	NULL	NULL	NULL	NULL	incidence	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the high incidence and severity of concurrent diabetes and amoeba , prophylactic measures are necessary for diabetic patients traveling in developing countries .
	manualset3
264337	2	424226	15	NULL	NULL	NULL	NULL	severity of concurrent diabetes	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the high incidence and severity of concurrent diabetes and amoeba , prophylactic measures are necessary for diabetic patients traveling in developing countries .
	manualset3
264338	3	424226	15	NULL	NULL	NULL	NULL	amoeba	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the high incidence and severity of concurrent diabetes and amoeba , prophylactic measures are necessary for diabetic patients traveling in developing countries .
	manualset3
264339	4	424226	15	NULL	NULL	NULL	NULL	prophylactic measures	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the high incidence and severity of concurrent diabetes and amoeba , prophylactic measures are necessary for diabetic patients traveling in developing countries .
	manualset3
264340	5	424226	15	NULL	NULL	NULL	NULL	diabetic patients 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the high incidence and severity of concurrent diabetes and amoeba , prophylactic measures are necessary for diabetic patients traveling in developing countries .
	manualset3
264341	6	424226	15	NULL	NULL	NULL	NULL	developing countries	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the high incidence and severity of concurrent diabetes and amoeba , prophylactic measures are necessary for diabetic patients traveling in developing countries .
	manualset3
264342	1	424227	15	NULL	NULL	NULL	NULL	variability	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the important variability in US measurement of kidney length it is not possible to definitely conclude that length and growth curve of kidneys in madagascan children are statistically different from those of the published normative standards .
	manualset3
264343	2	424227	15	NULL	NULL	NULL	NULL	US measurement	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the important variability in US measurement of kidney length it is not possible to definitely conclude that length and growth curve of kidneys in madagascan children are statistically different from those of the published normative standards .
	manualset3
264345	3	424227	15	NULL	NULL	NULL	NULL	kidney length	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the important variability in US measurement of kidney length it is not possible to definitely conclude that length and growth curve of kidneys in madagascan children are statistically different from those of the published normative standards .
	manualset3
264346	4	424227	15	NULL	NULL	NULL	NULL	length	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the important variability in US measurement of kidney length it is not possible to definitely conclude that length and growth curve of kidneys in madagascan children are statistically different from those of the published normative standards .
	manualset3
264347	5	424227	15	NULL	NULL	NULL	NULL	growth curve 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the important variability in US measurement of kidney length it is not possible to definitely conclude that length and growth curve of kidneys in madagascan children are statistically different from those of the published normative standards .
	manualset3
264348	6	424227	15	NULL	NULL	NULL	NULL	kidneys 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the important variability in US measurement of kidney length it is not possible to definitely conclude that length and growth curve of kidneys in madagascan children are statistically different from those of the published normative standards .
	manualset3
264349	7	424227	15	NULL	NULL	NULL	NULL	madagascan children 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the important variability in US measurement of kidney length it is not possible to definitely conclude that length and growth curve of kidneys in madagascan children are statistically different from those of the published normative standards .
	manualset3
264350	8	424227	15	NULL	NULL	NULL	NULL	published normative standards	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the important variability in US measurement of kidney length it is not possible to definitely conclude that length and growth curve of kidneys in madagascan children are statistically different from those of the published normative standards .
	manualset3
264351	1	424228	15	NULL	NULL	NULL	NULL	intraindividual variability	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the intraindividual variability in the pharmacokinetics of terfenadine , further study is needed to confirm these results .
	manualset3
264352	2	424228	15	NULL	NULL	NULL	NULL	pharmacokinetics 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the intraindividual variability in the pharmacokinetics of terfenadine , further study is needed to confirm these results .
	manualset3
264353	3	424228	15	NULL	NULL	NULL	NULL	terfenadine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the intraindividual variability in the pharmacokinetics of terfenadine , further study is needed to confirm these results .
	manualset3
264354	4	424228	15	NULL	NULL	NULL	NULL	 study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the intraindividual variability in the pharmacokinetics of terfenadine , further study is needed to confirm these results .
	manualset3
264355	5	424228	15	NULL	NULL	NULL	NULL	results	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the intraindividual variability in the pharmacokinetics of terfenadine , further study is needed to confirm these results .
	manualset3
264356	1	424229	15	NULL	NULL	NULL	NULL	Expression 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Expression of the p53 protein in human osteosarcoma ) .
	manualset3
264357	2	424229	15	NULL	NULL	NULL	NULL	p53 protein	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Expression of the p53 protein in human osteosarcoma ) .
	manualset3
264358	3	424229	15	NULL	NULL	NULL	NULL	human osteosarcoma 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Expression of the p53 protein in human osteosarcoma ) .
	manualset3
264359	1	424230	15	NULL	NULL	NULL	NULL	variations	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the large variations between different sieve tubes and different plants , the nutrient delivery to sink tissues is not homeostatic over time .
	manualset3
264360	2	424230	15	NULL	NULL	NULL	NULL	sieve tubes	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the large variations between different sieve tubes and different plants , the nutrient delivery to sink tissues is not homeostatic over time .
	manualset3
264361	3	424230	15	NULL	NULL	NULL	NULL	plants	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the large variations between different sieve tubes and different plants , the nutrient delivery to sink tissues is not homeostatic over time .
	manualset3
264362	4	424230	15	NULL	NULL	NULL	NULL	nutrient delivery	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the large variations between different sieve tubes and different plants , the nutrient delivery to sink tissues is not homeostatic over time .
	manualset3
264363	5	424230	15	NULL	NULL	NULL	NULL	sink tissues	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the large variations between different sieve tubes and different plants , the nutrient delivery to sink tissues is not homeostatic over time .
	manualset3
264364	6	424230	15	NULL	NULL	NULL	NULL	over time	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the large variations between different sieve tubes and different plants , the nutrient delivery to sink tissues is not homeostatic over time .
	manualset3
264365	1	424231	15	NULL	NULL	NULL	NULL	parallel roles	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the parallel roles and physical proximity of Mac-1 and uPAR , the capacity of these receptors to functionally interact was explored .
	manualset3
264366	2	424231	15	NULL	NULL	NULL	NULL	physical proximity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the parallel roles and physical proximity of Mac-1 and uPAR , the capacity of these receptors to functionally interact was explored .
	manualset3
264367	3	424231	15	NULL	NULL	NULL	NULL	Mac-1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the parallel roles and physical proximity of Mac-1 and uPAR , the capacity of these receptors to functionally interact was explored .
	manualset3
264368	4	424231	15	NULL	NULL	NULL	NULL	uPAR 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the parallel roles and physical proximity of Mac-1 and uPAR , the capacity of these receptors to functionally interact was explored .
	manualset3
264369	5	424231	15	NULL	NULL	NULL	NULL	capacity	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the parallel roles and physical proximity of Mac-1 and uPAR , the capacity of these receptors to functionally interact was explored .
	manualset3
264370	6	424231	15	NULL	NULL	NULL	NULL	receptors	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the parallel roles and physical proximity of Mac-1 and uPAR , the capacity of these receptors to functionally interact was explored .
	manualset3
264371	1	424232	15	NULL	NULL	NULL	NULL	relatively fast rate 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the relatively fast rate of plasmid DNA cleavage , an observed rate constant of ( 1.2 0.5 ) 10 ( -5 ) s ( -1 ) for cleavage of form II DNA to form III was also able to be determined .
	manualset3
264372	2	424232	15	NULL	NULL	NULL	NULL	plasmid DNA cleavage	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the relatively fast rate of plasmid DNA cleavage , an observed rate constant of ( 1.2 0.5 ) 10 ( -5 ) s ( -1 ) for cleavage of form II DNA to form III was also able to be determined .
	manualset3
264373	3	424232	15	NULL	NULL	NULL	NULL	observed rate constant	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the relatively fast rate of plasmid DNA cleavage , an observed rate constant of ( 1.2 0.5 ) 10 ( -5 ) s ( -1 ) for cleavage of form II DNA to form III was also able to be determined .
	manualset3
264374	4	424232	15	NULL	NULL	NULL	NULL	( 1.2 0.5 ) 10 ( -5 ) s ( -1 )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the relatively fast rate of plasmid DNA cleavage , an observed rate constant of ( 1.2 0.5 ) 10 ( -5 ) s ( -1 ) for cleavage of form II DNA to form III was also able to be determined .
	manualset3
264375	5	424232	15	NULL	NULL	NULL	NULL	cleavage	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the relatively fast rate of plasmid DNA cleavage , an observed rate constant of ( 1.2 0.5 ) 10 ( -5 ) s ( -1 ) for cleavage of form II DNA to form III was also able to be determined .
	manualset3
264376	6	424232	15	NULL	NULL	NULL	NULL	form II DNA	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the relatively fast rate of plasmid DNA cleavage , an observed rate constant of ( 1.2 0.5 ) 10 ( -5 ) s ( -1 ) for cleavage of form II DNA to form III was also able to be determined .
	manualset3
264377	7	424232	15	NULL	NULL	NULL	NULL	form III 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the relatively fast rate of plasmid DNA cleavage , an observed rate constant of ( 1.2 0.5 ) 10 ( -5 ) s ( -1 ) for cleavage of form II DNA to form III was also able to be determined .
	manualset3
264378	1	424233	15	NULL	NULL	NULL	NULL	special features	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the special features of subdental synchondrosis , fracture of the odontoid process in childhood can be seen as a separate entity .
	manualset3
264379	2	424233	15	NULL	NULL	NULL	NULL	subdental synchondrosis	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the special features of subdental synchondrosis , fracture of the odontoid process in childhood can be seen as a separate entity .
	manualset3
264380	3	424233	15	NULL	NULL	NULL	NULL	fracture	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the special features of subdental synchondrosis , fracture of the odontoid process in childhood can be seen as a separate entity .
	manualset3
264381	4	424233	15	NULL	NULL	NULL	NULL	odontoid process	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the special features of subdental synchondrosis , fracture of the odontoid process in childhood can be seen as a separate entity .
	manualset3
264382	5	424233	15	NULL	NULL	NULL	NULL	childhood	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the special features of subdental synchondrosis , fracture of the odontoid process in childhood can be seen as a separate entity .
	manualset3
264383	6	424233	15	NULL	NULL	NULL	NULL	entity	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the special features of subdental synchondrosis , fracture of the odontoid process in childhood can be seen as a separate entity .
	manualset3
264384	1	424234	15	NULL	NULL	NULL	NULL	substantial risk	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the substantial risk of thrombotic complications , elderly patients , ie , those older than 70 years , should be treated initially with phlebotomy and myelosuppressive therapy , usually 32P .
	manualset3
264385	3	424234	15	NULL	NULL	NULL	NULL	elderly patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the substantial risk of thrombotic complications , elderly patients , ie , those older than 70 years , should be treated initially with phlebotomy and myelosuppressive therapy , usually 32P .
	manualset3
264386	4	424234	15	NULL	NULL	NULL	NULL	70 years	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the substantial risk of thrombotic complications , elderly patients , ie , those older than 70 years , should be treated initially with phlebotomy and myelosuppressive therapy , usually 32P .
	manualset3
264387	5	424234	15	NULL	NULL	NULL	NULL	phlebotomy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the substantial risk of thrombotic complications , elderly patients , ie , those older than 70 years , should be treated initially with phlebotomy and myelosuppressive therapy , usually 32P .
	manualset3
264388	6	424234	15	NULL	NULL	NULL	NULL	myelosuppressive therapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the substantial risk of thrombotic complications , elderly patients , ie , those older than 70 years , should be treated initially with phlebotomy and myelosuppressive therapy , usually 32P .
	manualset3
264389	7	424234	15	NULL	NULL	NULL	NULL	32P	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the substantial risk of thrombotic complications , elderly patients , ie , those older than 70 years , should be treated initially with phlebotomy and myelosuppressive therapy , usually 32P .
	manualset3
264390	2	424234	15	NULL	NULL	NULL	NULL	thrombotic complications	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of the substantial risk of thrombotic complications , elderly patients , ie , those older than 70 years , should be treated initially with phlebotomy and myelosuppressive therapy , usually 32P .
	manualset3
264391	1	424235	15	NULL	NULL	NULL	NULL	slow turnover rates	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of these slow turnover rates , carbon and nitrogen stable isotope analysis in manatee epidermis is useful in summarizing average dietary intake over a long period of time rather than assessing recent diet .
	manualset3
264392	2	424235	15	NULL	NULL	NULL	NULL	carbon	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of these slow turnover rates , carbon and nitrogen stable isotope analysis in manatee epidermis is useful in summarizing average dietary intake over a long period of time rather than assessing recent diet .
	manualset3
264393	3	424235	15	NULL	NULL	NULL	NULL	 nitrogen 	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of these slow turnover rates , carbon and nitrogen stable isotope analysis in manatee epidermis is useful in summarizing average dietary intake over a long period of time rather than assessing recent diet .
	manualset3
264394	4	424235	15	NULL	NULL	NULL	NULL	stable isotope analysis 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of these slow turnover rates , carbon and nitrogen stable isotope analysis in manatee epidermis is useful in summarizing average dietary intake over a long period of time rather than assessing recent diet .
	manualset3
264395	5	424235	15	NULL	NULL	NULL	NULL	manatee epidermis	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of these slow turnover rates , carbon and nitrogen stable isotope analysis in manatee epidermis is useful in summarizing average dietary intake over a long period of time rather than assessing recent diet .
	manualset3
264396	6	424235	15	NULL	NULL	NULL	NULL	average dietary intake	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of these slow turnover rates , carbon and nitrogen stable isotope analysis in manatee epidermis is useful in summarizing average dietary intake over a long period of time rather than assessing recent diet .
	manualset3
264397	7	424235	15	NULL	NULL	NULL	NULL	long period of time	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of these slow turnover rates , carbon and nitrogen stable isotope analysis in manatee epidermis is useful in summarizing average dietary intake over a long period of time rather than assessing recent diet .
	manualset3
264398	8	424235	15	NULL	NULL	NULL	NULL	diet	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of these slow turnover rates , carbon and nitrogen stable isotope analysis in manatee epidermis is useful in summarizing average dietary intake over a long period of time rather than assessing recent diet .
	manualset3
264399	1	424236	15	NULL	NULL	NULL	NULL	Extracorporeal lung support	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Extracorporeal lung support in patients with severe respiratory failure secondary to the 2010-2011 winter seasonal outbreak of influenza A ( H1N1 ) in Spain ) .
	manualset3
264400	2	424236	15	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Extracorporeal lung support in patients with severe respiratory failure secondary to the 2010-2011 winter seasonal outbreak of influenza A ( H1N1 ) in Spain ) .
	manualset3
264401	3	424236	15	NULL	NULL	NULL	NULL	 severe respiratory failure	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Extracorporeal lung support in patients with severe respiratory failure secondary to the 2010-2011 winter seasonal outbreak of influenza A ( H1N1 ) in Spain ) .
	manualset3
264402	4	424236	15	NULL	NULL	NULL	NULL	2010-2011 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Extracorporeal lung support in patients with severe respiratory failure secondary to the 2010-2011 winter seasonal outbreak of influenza A ( H1N1 ) in Spain ) .
	manualset3
264403	5	424236	15	NULL	NULL	NULL	NULL	winter seasonal outbreak 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Extracorporeal lung support in patients with severe respiratory failure secondary to the 2010-2011 winter seasonal outbreak of influenza A ( H1N1 ) in Spain ) .
	manualset3
264404	6	424236	15	NULL	NULL	NULL	NULL	influenza A ( H1N1 ) 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Extracorporeal lung support in patients with severe respiratory failure secondary to the 2010-2011 winter seasonal outbreak of influenza A ( H1N1 ) in Spain ) .
	manualset3
264405	7	424236	15	NULL	NULL	NULL	NULL	Spain	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Extracorporeal lung support in patients with severe respiratory failure secondary to the 2010-2011 winter seasonal outbreak of influenza A ( H1N1 ) in Spain ) .
	manualset3
264406	1	424237	15	NULL	NULL	NULL	NULL	two observations	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of these two observations , LRRK2 has been intensively investigated for its pathogenic mechanism ( s ) and as a target gene for PD therapeutics .
	manualset3
264407	2	424237	15	NULL	NULL	NULL	NULL	LRRK2	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of these two observations , LRRK2 has been intensively investigated for its pathogenic mechanism ( s ) and as a target gene for PD therapeutics .
	manualset3
264408	3	424237	15	NULL	NULL	NULL	NULL	pathogenic mechanism ( s ) 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of these two observations , LRRK2 has been intensively investigated for its pathogenic mechanism ( s ) and as a target gene for PD therapeutics .
	manualset3
264409	4	424237	15	NULL	NULL	NULL	NULL	target gene	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of these two observations , LRRK2 has been intensively investigated for its pathogenic mechanism ( s ) and as a target gene for PD therapeutics .
	manualset3
264410	5	424237	15	NULL	NULL	NULL	NULL	PD therapeutics	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because of these two observations , LRRK2 has been intensively investigated for its pathogenic mechanism ( s ) and as a target gene for PD therapeutics .
	manualset3
264411	1	424238	15	NULL	NULL	NULL	NULL	optimal therapeutic strategies	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because optimal therapeutic strategies vary with tumor type , an accurate diagnosis is the foundation of enlightened management decisions .
	manualset3
264412	2	424238	15	NULL	NULL	NULL	NULL	tumor type	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because optimal therapeutic strategies vary with tumor type , an accurate diagnosis is the foundation of enlightened management decisions .
	manualset3
264413	3	424238	15	NULL	NULL	NULL	NULL	accurate diagnosis	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because optimal therapeutic strategies vary with tumor type , an accurate diagnosis is the foundation of enlightened management decisions .
	manualset3
264414	4	424238	15	NULL	NULL	NULL	NULL	foundation	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because optimal therapeutic strategies vary with tumor type , an accurate diagnosis is the foundation of enlightened management decisions .
	manualset3
264415	5	424238	15	NULL	NULL	NULL	NULL	management decisions	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because optimal therapeutic strategies vary with tumor type , an accurate diagnosis is the foundation of enlightened management decisions .
	manualset3
264416	1	424239	15	NULL	NULL	NULL	NULL	oxidants 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because oxidants are the major mechanism of smoking-induced airway damage , we hypothesized that smoking is associated with upregulation of various antioxidant-related genes in the airway epithelium , but the magnitude of the response shows high inter-individual variability .
	manualset3
264417	2	424239	15	NULL	NULL	NULL	NULL	mechanism	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because oxidants are the major mechanism of smoking-induced airway damage , we hypothesized that smoking is associated with upregulation of various antioxidant-related genes in the airway epithelium , but the magnitude of the response shows high inter-individual variability .
	manualset3
264418	3	424239	15	NULL	NULL	NULL	NULL	smoking-induced airway damage	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because oxidants are the major mechanism of smoking-induced airway damage , we hypothesized that smoking is associated with upregulation of various antioxidant-related genes in the airway epithelium , but the magnitude of the response shows high inter-individual variability .
	manualset3
264419	4	424239	15	NULL	NULL	NULL	NULL	smoking	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because oxidants are the major mechanism of smoking-induced airway damage , we hypothesized that smoking is associated with upregulation of various antioxidant-related genes in the airway epithelium , but the magnitude of the response shows high inter-individual variability .
	manualset3
264420	5	424239	15	NULL	NULL	NULL	NULL	upregulation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because oxidants are the major mechanism of smoking-induced airway damage , we hypothesized that smoking is associated with upregulation of various antioxidant-related genes in the airway epithelium , but the magnitude of the response shows high inter-individual variability .
	manualset3
264421	6	424239	15	NULL	NULL	NULL	NULL	antioxidant-related genes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because oxidants are the major mechanism of smoking-induced airway damage , we hypothesized that smoking is associated with upregulation of various antioxidant-related genes in the airway epithelium , but the magnitude of the response shows high inter-individual variability .
	manualset3
264422	7	424239	15	NULL	NULL	NULL	NULL	airway epithelium	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because oxidants are the major mechanism of smoking-induced airway damage , we hypothesized that smoking is associated with upregulation of various antioxidant-related genes in the airway epithelium , but the magnitude of the response shows high inter-individual variability .
	manualset3
264423	8	424239	15	NULL	NULL	NULL	NULL	 magnitude of the response	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because oxidants are the major mechanism of smoking-induced airway damage , we hypothesized that smoking is associated with upregulation of various antioxidant-related genes in the airway epithelium , but the magnitude of the response shows high inter-individual variability .
	manualset3
264424	9	424239	15	NULL	NULL	NULL	NULL	high inter-individual variability	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because oxidants are the major mechanism of smoking-induced airway damage , we hypothesized that smoking is associated with upregulation of various antioxidant-related genes in the airway epithelium , but the magnitude of the response shows high inter-individual variability .
	manualset3
264425	1	424240	15	NULL	NULL	NULL	NULL	oxygen tensions	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because oxygen tensions in human body differ from one tissue to another and change depending on their metabolism , biological activity of NO in various tissues might be affected by local oxygen tensions .
	manualset3
264426	2	424240	15	NULL	NULL	NULL	NULL	human body	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because oxygen tensions in human body differ from one tissue to another and change depending on their metabolism , biological activity of NO in various tissues might be affected by local oxygen tensions .
	manualset3
264427	3	424240	15	NULL	NULL	NULL	NULL	one	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because oxygen tensions in human body differ from one tissue to another and change depending on their metabolism , biological activity of NO in various tissues might be affected by local oxygen tensions .
	manualset3
264428	4	424240	15	NULL	NULL	NULL	NULL	tissue	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because oxygen tensions in human body differ from one tissue to another and change depending on their metabolism , biological activity of NO in various tissues might be affected by local oxygen tensions .
	manualset3
264656	5	424240	15	NULL	NULL	NULL	NULL	change	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because oxygen tensions in human body differ from one tissue to another and change depending on their metabolism , biological activity of NO in various tissues might be affected by local oxygen tensions .
	manualset3
264657	6	424240	15	NULL	NULL	NULL	NULL	metabolism	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because oxygen tensions in human body differ from one tissue to another and change depending on their metabolism , biological activity of NO in various tissues might be affected by local oxygen tensions .
	manualset3
264658	7	424240	15	NULL	NULL	NULL	NULL	biological activity of NO	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because oxygen tensions in human body differ from one tissue to another and change depending on their metabolism , biological activity of NO in various tissues might be affected by local oxygen tensions .
	manualset3
264659	8	424240	15	NULL	NULL	NULL	NULL	tissues 	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because oxygen tensions in human body differ from one tissue to another and change depending on their metabolism , biological activity of NO in various tissues might be affected by local oxygen tensions .
	manualset3
264661	9	424240	15	NULL	NULL	NULL	NULL	oxygen tensions	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because oxygen tensions in human body differ from one tissue to another and change depending on their metabolism , biological activity of NO in various tissues might be affected by local oxygen tensions .
	manualset3
264666	1	424241	15	NULL	NULL	NULL	NULL	patients 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because patients with undiagnosed APRT deficiency who undergo kidney transplant may risk losing the transplant because of an otherwise treatable disease , increased physician awareness may hasten the diagnosis and limit the morbidity associated with this disease .
	manualset3
264667	2	424241	15	NULL	NULL	NULL	NULL	APRT deficiency	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because patients with undiagnosed APRT deficiency who undergo kidney transplant may risk losing the transplant because of an otherwise treatable disease , increased physician awareness may hasten the diagnosis and limit the morbidity associated with this disease .
	manualset3
264668	3	424241	15	NULL	NULL	NULL	NULL	kidney transplant	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because patients with undiagnosed APRT deficiency who undergo kidney transplant may risk losing the transplant because of an otherwise treatable disease , increased physician awareness may hasten the diagnosis and limit the morbidity associated with this disease .
	manualset3
264669	4	424241	15	NULL	NULL	NULL	NULL	transplant 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because patients with undiagnosed APRT deficiency who undergo kidney transplant may risk losing the transplant because of an otherwise treatable disease , increased physician awareness may hasten the diagnosis and limit the morbidity associated with this disease .
	manualset3
264671	5	424241	15	NULL	NULL	NULL	NULL	treatable disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because patients with undiagnosed APRT deficiency who undergo kidney transplant may risk losing the transplant because of an otherwise treatable disease , increased physician awareness may hasten the diagnosis and limit the morbidity associated with this disease .
	manualset3
264675	6	424241	15	NULL	NULL	NULL	NULL	physician 	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because patients with undiagnosed APRT deficiency who undergo kidney transplant may risk losing the transplant because of an otherwise treatable disease , increased physician awareness may hasten the diagnosis and limit the morbidity associated with this disease .
	manualset3
264676	7	424241	15	NULL	NULL	NULL	NULL	awareness	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because patients with undiagnosed APRT deficiency who undergo kidney transplant may risk losing the transplant because of an otherwise treatable disease , increased physician awareness may hasten the diagnosis and limit the morbidity associated with this disease .
	manualset3
264677	8	424241	15	NULL	NULL	NULL	NULL	diagnosis 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because patients with undiagnosed APRT deficiency who undergo kidney transplant may risk losing the transplant because of an otherwise treatable disease , increased physician awareness may hasten the diagnosis and limit the morbidity associated with this disease .
	manualset3
264679	9	424241	15	NULL	NULL	NULL	NULL	limit	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because patients with undiagnosed APRT deficiency who undergo kidney transplant may risk losing the transplant because of an otherwise treatable disease , increased physician awareness may hasten the diagnosis and limit the morbidity associated with this disease .
	manualset3
264681	10	424241	15	NULL	NULL	NULL	NULL	morbidity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because patients with undiagnosed APRT deficiency who undergo kidney transplant may risk losing the transplant because of an otherwise treatable disease , increased physician awareness may hasten the diagnosis and limit the morbidity associated with this disease .
	manualset3
264682	11	424241	15	NULL	NULL	NULL	NULL	disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because patients with undiagnosed APRT deficiency who undergo kidney transplant may risk losing the transplant because of an otherwise treatable disease , increased physician awareness may hasten the diagnosis and limit the morbidity associated with this disease .
	manualset3
264693	1	424242	15	NULL	NULL	NULL	NULL	phosphorylation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because phosphorylation of TRPV1 ( transient receptor potential subtype V1 ) plays a key role in the induction of thermal hyperalgesia in inflammatory pain models , we evaluated whether the cannabinoid agonist WIN 55 , 212-2 ( WIN ) regulates the phosphorylation state of TRPV1 .
	manualset3
264696	2	424242	15	NULL	NULL	NULL	NULL	TRPV1 ( transient receptor potential subtype V1 ) 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because phosphorylation of TRPV1 ( transient receptor potential subtype V1 ) plays a key role in the induction of thermal hyperalgesia in inflammatory pain models , we evaluated whether the cannabinoid agonist WIN 55 , 212-2 ( WIN ) regulates the phosphorylation state of TRPV1 .
	manualset3
264697	3	424242	15	NULL	NULL	NULL	NULL	role	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because phosphorylation of TRPV1 ( transient receptor potential subtype V1 ) plays a key role in the induction of thermal hyperalgesia in inflammatory pain models , we evaluated whether the cannabinoid agonist WIN 55 , 212-2 ( WIN ) regulates the phosphorylation state of TRPV1 .
	manualset3
264703	4	424242	15	NULL	NULL	NULL	NULL	induction of thermal hyperalgesia	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because phosphorylation of TRPV1 ( transient receptor potential subtype V1 ) plays a key role in the induction of thermal hyperalgesia in inflammatory pain models , we evaluated whether the cannabinoid agonist WIN 55 , 212-2 ( WIN ) regulates the phosphorylation state of TRPV1 .
	manualset3
264706	5	424242	15	NULL	NULL	NULL	NULL	inflammatory pain models	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because phosphorylation of TRPV1 ( transient receptor potential subtype V1 ) plays a key role in the induction of thermal hyperalgesia in inflammatory pain models , we evaluated whether the cannabinoid agonist WIN 55 , 212-2 ( WIN ) regulates the phosphorylation state of TRPV1 .
	manualset3
264708	6	424242	15	NULL	NULL	NULL	NULL	cannabinoid agonist WIN 55	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because phosphorylation of TRPV1 ( transient receptor potential subtype V1 ) plays a key role in the induction of thermal hyperalgesia in inflammatory pain models , we evaluated whether the cannabinoid agonist WIN 55 , 212-2 ( WIN ) regulates the phosphorylation state of TRPV1 .
	manualset3
264710	7	424242	15	NULL	NULL	NULL	NULL	212-2 ( WIN ) 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because phosphorylation of TRPV1 ( transient receptor potential subtype V1 ) plays a key role in the induction of thermal hyperalgesia in inflammatory pain models , we evaluated whether the cannabinoid agonist WIN 55 , 212-2 ( WIN ) regulates the phosphorylation state of TRPV1 .
	manualset3
264712	8	424242	15	NULL	NULL	NULL	NULL	phosphorylation state 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because phosphorylation of TRPV1 ( transient receptor potential subtype V1 ) plays a key role in the induction of thermal hyperalgesia in inflammatory pain models , we evaluated whether the cannabinoid agonist WIN 55 , 212-2 ( WIN ) regulates the phosphorylation state of TRPV1 .
	manualset3
264713	9	424242	15	NULL	NULL	NULL	NULL	TRPV1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because phosphorylation of TRPV1 ( transient receptor potential subtype V1 ) plays a key role in the induction of thermal hyperalgesia in inflammatory pain models , we evaluated whether the cannabinoid agonist WIN 55 , 212-2 ( WIN ) regulates the phosphorylation state of TRPV1 .
	manualset3
264715	1	424243	15	NULL	NULL	NULL	NULL	protein functions	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because protein functions are generally determined by its structure , molecular dynamics simulations were performed in this study to understand the structure and its stability of a 66-amino acid fragment of a group 3 LEA protein from an anhydrobiotic nematode during desiccation .
	manualset3
264717	2	424243	15	NULL	NULL	NULL	NULL	structure	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because protein functions are generally determined by its structure , molecular dynamics simulations were performed in this study to understand the structure and its stability of a 66-amino acid fragment of a group 3 LEA protein from an anhydrobiotic nematode during desiccation .
	manualset3
264718	3	424243	15	NULL	NULL	NULL	NULL	molecular dynamics simulations	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because protein functions are generally determined by its structure , molecular dynamics simulations were performed in this study to understand the structure and its stability of a 66-amino acid fragment of a group 3 LEA protein from an anhydrobiotic nematode during desiccation .
	manualset3
264720	4	424243	15	NULL	NULL	NULL	NULL	study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because protein functions are generally determined by its structure , molecular dynamics simulations were performed in this study to understand the structure and its stability of a 66-amino acid fragment of a group 3 LEA protein from an anhydrobiotic nematode during desiccation .
	manualset3
264723	5	424243	15	NULL	NULL	NULL	NULL	structure	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because protein functions are generally determined by its structure , molecular dynamics simulations were performed in this study to understand the structure and its stability of a 66-amino acid fragment of a group 3 LEA protein from an anhydrobiotic nematode during desiccation .
	manualset3
264724	6	424243	15	NULL	NULL	NULL	NULL	stability	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because protein functions are generally determined by its structure , molecular dynamics simulations were performed in this study to understand the structure and its stability of a 66-amino acid fragment of a group 3 LEA protein from an anhydrobiotic nematode during desiccation .
	manualset3
264726	7	424243	15	NULL	NULL	NULL	NULL	66-amino acid fragment 	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because protein functions are generally determined by its structure , molecular dynamics simulations were performed in this study to understand the structure and its stability of a 66-amino acid fragment of a group 3 LEA protein from an anhydrobiotic nematode during desiccation .
	manualset3
264727	8	424243	15	NULL	NULL	NULL	NULL	group 3 LEA protein	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because protein functions are generally determined by its structure , molecular dynamics simulations were performed in this study to understand the structure and its stability of a 66-amino acid fragment of a group 3 LEA protein from an anhydrobiotic nematode during desiccation .
	manualset3
264728	9	424243	15	NULL	NULL	NULL	NULL	anhydrobiotic nematode	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because protein functions are generally determined by its structure , molecular dynamics simulations were performed in this study to understand the structure and its stability of a 66-amino acid fragment of a group 3 LEA protein from an anhydrobiotic nematode during desiccation .
	manualset3
264729	10	424243	15	NULL	NULL	NULL	NULL	desiccation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because protein functions are generally determined by its structure , molecular dynamics simulations were performed in this study to understand the structure and its stability of a 66-amino acid fragment of a group 3 LEA protein from an anhydrobiotic nematode during desiccation .
	manualset3
264730	1	424244	15	NULL	NULL	NULL	NULL	pulp cells 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because pulp cells and periodontal ligament ( PDL ) fibroblasts can express thrombin receptor mRNA , the specific aim of this study was to determine whether thrombin can activate the growth , attachment , protein synthesis , alkaline phosphatase activities and cellular clustering of cultured human PDL fibroblasts .
	manualset3
264731	2	424244	15	NULL	NULL	NULL	NULL	periodontal ligament ( PDL ) fibroblasts	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because pulp cells and periodontal ligament ( PDL ) fibroblasts can express thrombin receptor mRNA , the specific aim of this study was to determine whether thrombin can activate the growth , attachment , protein synthesis , alkaline phosphatase activities and cellular clustering of cultured human PDL fibroblasts .
	manualset3
264732	3	424244	15	NULL	NULL	NULL	NULL	thrombin receptor mRNA	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because pulp cells and periodontal ligament ( PDL ) fibroblasts can express thrombin receptor mRNA , the specific aim of this study was to determine whether thrombin can activate the growth , attachment , protein synthesis , alkaline phosphatase activities and cellular clustering of cultured human PDL fibroblasts .
	manualset3
264733	4	424244	15	NULL	NULL	NULL	NULL	specific aim	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because pulp cells and periodontal ligament ( PDL ) fibroblasts can express thrombin receptor mRNA , the specific aim of this study was to determine whether thrombin can activate the growth , attachment , protein synthesis , alkaline phosphatase activities and cellular clustering of cultured human PDL fibroblasts .
	manualset3
264734	5	424244	15	NULL	NULL	NULL	NULL	study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because pulp cells and periodontal ligament ( PDL ) fibroblasts can express thrombin receptor mRNA , the specific aim of this study was to determine whether thrombin can activate the growth , attachment , protein synthesis , alkaline phosphatase activities and cellular clustering of cultured human PDL fibroblasts .
	manualset3
264735	6	424244	15	NULL	NULL	NULL	NULL	thrombin 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because pulp cells and periodontal ligament ( PDL ) fibroblasts can express thrombin receptor mRNA , the specific aim of this study was to determine whether thrombin can activate the growth , attachment , protein synthesis , alkaline phosphatase activities and cellular clustering of cultured human PDL fibroblasts .
	manualset3
264736	7	424244	15	NULL	NULL	NULL	NULL	growth	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because pulp cells and periodontal ligament ( PDL ) fibroblasts can express thrombin receptor mRNA , the specific aim of this study was to determine whether thrombin can activate the growth , attachment , protein synthesis , alkaline phosphatase activities and cellular clustering of cultured human PDL fibroblasts .
	manualset3
264737	8	424244	15	NULL	NULL	NULL	NULL	attachment 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because pulp cells and periodontal ligament ( PDL ) fibroblasts can express thrombin receptor mRNA , the specific aim of this study was to determine whether thrombin can activate the growth , attachment , protein synthesis , alkaline phosphatase activities and cellular clustering of cultured human PDL fibroblasts .
	manualset3
264738	9	424244	15	NULL	NULL	NULL	NULL	protein synthesis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because pulp cells and periodontal ligament ( PDL ) fibroblasts can express thrombin receptor mRNA , the specific aim of this study was to determine whether thrombin can activate the growth , attachment , protein synthesis , alkaline phosphatase activities and cellular clustering of cultured human PDL fibroblasts .
	manualset3
264739	10	424244	15	NULL	NULL	NULL	NULL	alkaline phosphatase activities	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because pulp cells and periodontal ligament ( PDL ) fibroblasts can express thrombin receptor mRNA , the specific aim of this study was to determine whether thrombin can activate the growth , attachment , protein synthesis , alkaline phosphatase activities and cellular clustering of cultured human PDL fibroblasts .
	manualset3
264740	11	424244	15	NULL	NULL	NULL	NULL	cellular clustering 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because pulp cells and periodontal ligament ( PDL ) fibroblasts can express thrombin receptor mRNA , the specific aim of this study was to determine whether thrombin can activate the growth , attachment , protein synthesis , alkaline phosphatase activities and cellular clustering of cultured human PDL fibroblasts .
	manualset3
264741	12	424244	15	NULL	NULL	NULL	NULL	cultured human PDL fibroblasts 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because pulp cells and periodontal ligament ( PDL ) fibroblasts can express thrombin receptor mRNA , the specific aim of this study was to determine whether thrombin can activate the growth , attachment , protein synthesis , alkaline phosphatase activities and cellular clustering of cultured human PDL fibroblasts .
	manualset3
264742	1	424245	15	NULL	NULL	NULL	NULL	recent studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because recent studies indicate an antiangiopathic effect of celiprolol , but not of metoprolol , in type 1 diabetes , we investigated the direct influence of exposure to high D-glucose concentrations on endothelial cells and the possible effects of both beta-blockers .
	manualset3
264743	2	424245	15	NULL	NULL	NULL	NULL	antiangiopathic effect	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because recent studies indicate an antiangiopathic effect of celiprolol , but not of metoprolol , in type 1 diabetes , we investigated the direct influence of exposure to high D-glucose concentrations on endothelial cells and the possible effects of both beta-blockers .
	manualset3
264744	3	424245	15	NULL	NULL	NULL	NULL	celiprolol	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because recent studies indicate an antiangiopathic effect of celiprolol , but not of metoprolol , in type 1 diabetes , we investigated the direct influence of exposure to high D-glucose concentrations on endothelial cells and the possible effects of both beta-blockers .
	manualset3
264746	4	424245	15	NULL	NULL	NULL	NULL	metoprolol 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because recent studies indicate an antiangiopathic effect of celiprolol , but not of metoprolol , in type 1 diabetes , we investigated the direct influence of exposure to high D-glucose concentrations on endothelial cells and the possible effects of both beta-blockers .
	manualset3
264747	5	424245	15	NULL	NULL	NULL	NULL	type 1 diabetes	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because recent studies indicate an antiangiopathic effect of celiprolol , but not of metoprolol , in type 1 diabetes , we investigated the direct influence of exposure to high D-glucose concentrations on endothelial cells and the possible effects of both beta-blockers .
	manualset3
264748	6	424245	15	NULL	NULL	NULL	NULL	direct influence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because recent studies indicate an antiangiopathic effect of celiprolol , but not of metoprolol , in type 1 diabetes , we investigated the direct influence of exposure to high D-glucose concentrations on endothelial cells and the possible effects of both beta-blockers .
	manualset3
264749	7	424245	15	NULL	NULL	NULL	NULL	exposure	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because recent studies indicate an antiangiopathic effect of celiprolol , but not of metoprolol , in type 1 diabetes , we investigated the direct influence of exposure to high D-glucose concentrations on endothelial cells and the possible effects of both beta-blockers .
	manualset3
264751	8	424245	15	NULL	NULL	NULL	NULL	high D-glucose concentrations 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because recent studies indicate an antiangiopathic effect of celiprolol , but not of metoprolol , in type 1 diabetes , we investigated the direct influence of exposure to high D-glucose concentrations on endothelial cells and the possible effects of both beta-blockers .
	manualset3
264753	9	424245	15	NULL	NULL	NULL	NULL	endothelial cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because recent studies indicate an antiangiopathic effect of celiprolol , but not of metoprolol , in type 1 diabetes , we investigated the direct influence of exposure to high D-glucose concentrations on endothelial cells and the possible effects of both beta-blockers .
	manualset3
264755	10	424245	15	NULL	NULL	NULL	NULL	 effects 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because recent studies indicate an antiangiopathic effect of celiprolol , but not of metoprolol , in type 1 diabetes , we investigated the direct influence of exposure to high D-glucose concentrations on endothelial cells and the possible effects of both beta-blockers .
	manualset3
264757	11	424245	15	NULL	NULL	NULL	NULL	beta-blockers	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because recent studies indicate an antiangiopathic effect of celiprolol , but not of metoprolol , in type 1 diabetes , we investigated the direct influence of exposure to high D-glucose concentrations on endothelial cells and the possible effects of both beta-blockers .
	manualset3
264764	1	424246	15	NULL	NULL	NULL	NULL	expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the expression of GPC3 during human embryonic and fetal periods remains largely unknown , we investigated by immunohistochemistry its pattern of expression during four periods of human development covering the embryonic period ( P1 ) from 5 to 8 weeks of development , and the fetal periods ( P2 , P3 and P4 ) from 9 to 28 weeks of development .
	manualset3
264765	2	424246	15	NULL	NULL	NULL	NULL	GPC3 	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the expression of GPC3 during human embryonic and fetal periods remains largely unknown , we investigated by immunohistochemistry its pattern of expression during four periods of human development covering the embryonic period ( P1 ) from 5 to 8 weeks of development , and the fetal periods ( P2 , P3 and P4 ) from 9 to 28 weeks of development .
	manualset3
264768	3	424246	15	NULL	NULL	NULL	NULL	 human embryonic periods	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the expression of GPC3 during human embryonic and fetal periods remains largely unknown , we investigated by immunohistochemistry its pattern of expression during four periods of human development covering the embryonic period ( P1 ) from 5 to 8 weeks of development , and the fetal periods ( P2 , P3 and P4 ) from 9 to 28 weeks of development .
	manualset3
264770	4	424246	15	NULL	NULL	NULL	NULL	fetal periods	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the expression of GPC3 during human embryonic and fetal periods remains largely unknown , we investigated by immunohistochemistry its pattern of expression during four periods of human development covering the embryonic period ( P1 ) from 5 to 8 weeks of development , and the fetal periods ( P2 , P3 and P4 ) from 9 to 28 weeks of development .
	manualset3
264771	5	424246	15	NULL	NULL	NULL	NULL	immunohistochemistry	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the expression of GPC3 during human embryonic and fetal periods remains largely unknown , we investigated by immunohistochemistry its pattern of expression during four periods of human development covering the embryonic period ( P1 ) from 5 to 8 weeks of development , and the fetal periods ( P2 , P3 and P4 ) from 9 to 28 weeks of development .
	manualset3
264772	6	424246	15	NULL	NULL	NULL	NULL	pattern of expression 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the expression of GPC3 during human embryonic and fetal periods remains largely unknown , we investigated by immunohistochemistry its pattern of expression during four periods of human development covering the embryonic period ( P1 ) from 5 to 8 weeks of development , and the fetal periods ( P2 , P3 and P4 ) from 9 to 28 weeks of development .
	manualset3
264773	7	424246	15	NULL	NULL	NULL	NULL	four periods	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the expression of GPC3 during human embryonic and fetal periods remains largely unknown , we investigated by immunohistochemistry its pattern of expression during four periods of human development covering the embryonic period ( P1 ) from 5 to 8 weeks of development , and the fetal periods ( P2 , P3 and P4 ) from 9 to 28 weeks of development .
	manualset3
264774	8	424246	15	NULL	NULL	NULL	NULL	human development 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the expression of GPC3 during human embryonic and fetal periods remains largely unknown , we investigated by immunohistochemistry its pattern of expression during four periods of human development covering the embryonic period ( P1 ) from 5 to 8 weeks of development , and the fetal periods ( P2 , P3 and P4 ) from 9 to 28 weeks of development .
	manualset3
264775	9	424246	15	NULL	NULL	NULL	NULL	embryonic period ( P1 )	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the expression of GPC3 during human embryonic and fetal periods remains largely unknown , we investigated by immunohistochemistry its pattern of expression during four periods of human development covering the embryonic period ( P1 ) from 5 to 8 weeks of development , and the fetal periods ( P2 , P3 and P4 ) from 9 to 28 weeks of development .
	manualset3
264776	10	424246	15	NULL	NULL	NULL	NULL	5 to 8 weeks 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the expression of GPC3 during human embryonic and fetal periods remains largely unknown , we investigated by immunohistochemistry its pattern of expression during four periods of human development covering the embryonic period ( P1 ) from 5 to 8 weeks of development , and the fetal periods ( P2 , P3 and P4 ) from 9 to 28 weeks of development .
	manualset3
264777	11	424246	15	NULL	NULL	NULL	NULL	development	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the expression of GPC3 during human embryonic and fetal periods remains largely unknown , we investigated by immunohistochemistry its pattern of expression during four periods of human development covering the embryonic period ( P1 ) from 5 to 8 weeks of development , and the fetal periods ( P2 , P3 and P4 ) from 9 to 28 weeks of development .
	manualset3
264778	12	424246	15	NULL	NULL	NULL	NULL	fetal periods ( P2 , P3 and P4 ) 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the expression of GPC3 during human embryonic and fetal periods remains largely unknown , we investigated by immunohistochemistry its pattern of expression during four periods of human development covering the embryonic period ( P1 ) from 5 to 8 weeks of development , and the fetal periods ( P2 , P3 and P4 ) from 9 to 28 weeks of development .
	manualset3
264779	13	424246	15	NULL	NULL	NULL	NULL	9 to 28 weeks	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the expression of GPC3 during human embryonic and fetal periods remains largely unknown , we investigated by immunohistochemistry its pattern of expression during four periods of human development covering the embryonic period ( P1 ) from 5 to 8 weeks of development , and the fetal periods ( P2 , P3 and P4 ) from 9 to 28 weeks of development .
	manualset3
264780	14	424246	15	NULL	NULL	NULL	NULL	development	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the expression of GPC3 during human embryonic and fetal periods remains largely unknown , we investigated by immunohistochemistry its pattern of expression during four periods of human development covering the embryonic period ( P1 ) from 5 to 8 weeks of development , and the fetal periods ( P2 , P3 and P4 ) from 9 to 28 weeks of development .
	manualset3
264781	1	424247	15	NULL	NULL	NULL	NULL	Extralaryngeal causes 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Extralaryngeal causes of phonation disorders ) .
	manualset3
264782	2	424247	15	NULL	NULL	NULL	NULL	phonation disorders	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Extralaryngeal causes of phonation disorders ) .
	manualset3
264783	1	424248	15	NULL	NULL	NULL	NULL	inhibition	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the inhibition of glycerophosphate-dependent respiration by oleate was eliminated by added CoQ ( 3 ) , our data indicate that the activating effect of CoQ ( 3 ) is related to the release of the inhibitory effect of endogenous free fatty acids ( FFA ) .
	manualset3
264784	2	424248	15	NULL	NULL	NULL	NULL	glycerophosphate-dependent respiration 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the inhibition of glycerophosphate-dependent respiration by oleate was eliminated by added CoQ ( 3 ) , our data indicate that the activating effect of CoQ ( 3 ) is related to the release of the inhibitory effect of endogenous free fatty acids ( FFA ) .
	manualset3
264785	3	424248	15	NULL	NULL	NULL	NULL	oleate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the inhibition of glycerophosphate-dependent respiration by oleate was eliminated by added CoQ ( 3 ) , our data indicate that the activating effect of CoQ ( 3 ) is related to the release of the inhibitory effect of endogenous free fatty acids ( FFA ) .
	manualset3
264786	4	424248	15	NULL	NULL	NULL	NULL	CoQ ( 3 )	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the inhibition of glycerophosphate-dependent respiration by oleate was eliminated by added CoQ ( 3 ) , our data indicate that the activating effect of CoQ ( 3 ) is related to the release of the inhibitory effect of endogenous free fatty acids ( FFA ) .
	manualset3
264787	5	424248	15	NULL	NULL	NULL	NULL	data 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the inhibition of glycerophosphate-dependent respiration by oleate was eliminated by added CoQ ( 3 ) , our data indicate that the activating effect of CoQ ( 3 ) is related to the release of the inhibitory effect of endogenous free fatty acids ( FFA ) .
	manualset3
264788	6	424248	15	NULL	NULL	NULL	NULL	activating effect of CoQ ( 3 )	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the inhibition of glycerophosphate-dependent respiration by oleate was eliminated by added CoQ ( 3 ) , our data indicate that the activating effect of CoQ ( 3 ) is related to the release of the inhibitory effect of endogenous free fatty acids ( FFA ) .
	manualset3
264789	7	424248	15	NULL	NULL	NULL	NULL	release	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the inhibition of glycerophosphate-dependent respiration by oleate was eliminated by added CoQ ( 3 ) , our data indicate that the activating effect of CoQ ( 3 ) is related to the release of the inhibitory effect of endogenous free fatty acids ( FFA ) .
	manualset3
264790	8	424248	15	NULL	NULL	NULL	NULL	inhibitory effect	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the inhibition of glycerophosphate-dependent respiration by oleate was eliminated by added CoQ ( 3 ) , our data indicate that the activating effect of CoQ ( 3 ) is related to the release of the inhibitory effect of endogenous free fatty acids ( FFA ) .
	manualset3
264791	9	424248	15	NULL	NULL	NULL	NULL	endogenous free fatty acids ( FFA ) 	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the inhibition of glycerophosphate-dependent respiration by oleate was eliminated by added CoQ ( 3 ) , our data indicate that the activating effect of CoQ ( 3 ) is related to the release of the inhibitory effect of endogenous free fatty acids ( FFA ) .
	manualset3
264792	1	424249	15	NULL	NULL	NULL	NULL	ionic charge	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the ionic charge tends to remain localized on the sodium atom and because at least two bonds must be broken in order to produce polycyclic backbone fragmentation , it is extremely difficult to obtain abundant product ions ( other than Na + ) from ( M + Na ) + brevetoxin precursor ions in low-energy collision-induced dissociation ( CID ) MS/MS experiments .
	manualset3
264793	2	424249	15	NULL	NULL	NULL	NULL	sodium atom	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the ionic charge tends to remain localized on the sodium atom and because at least two bonds must be broken in order to produce polycyclic backbone fragmentation , it is extremely difficult to obtain abundant product ions ( other than Na + ) from ( M + Na ) + brevetoxin precursor ions in low-energy collision-induced dissociation ( CID ) MS/MS experiments .
	manualset3
264794	3	424249	15	NULL	NULL	NULL	NULL	two bonds 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the ionic charge tends to remain localized on the sodium atom and because at least two bonds must be broken in order to produce polycyclic backbone fragmentation , it is extremely difficult to obtain abundant product ions ( other than Na + ) from ( M + Na ) + brevetoxin precursor ions in low-energy collision-induced dissociation ( CID ) MS/MS experiments .
	manualset3
264795	4	424249	15	NULL	NULL	NULL	NULL	polycyclic backbone fragmentation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the ionic charge tends to remain localized on the sodium atom and because at least two bonds must be broken in order to produce polycyclic backbone fragmentation , it is extremely difficult to obtain abundant product ions ( other than Na + ) from ( M + Na ) + brevetoxin precursor ions in low-energy collision-induced dissociation ( CID ) MS/MS experiments .
	manualset3
264796	5	424249	15	NULL	NULL	NULL	NULL	abundant product ions 	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the ionic charge tends to remain localized on the sodium atom and because at least two bonds must be broken in order to produce polycyclic backbone fragmentation , it is extremely difficult to obtain abundant product ions ( other than Na + ) from ( M + Na ) + brevetoxin precursor ions in low-energy collision-induced dissociation ( CID ) MS/MS experiments .
	manualset3
264797	6	424249	15	NULL	NULL	NULL	NULL	Na + 	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the ionic charge tends to remain localized on the sodium atom and because at least two bonds must be broken in order to produce polycyclic backbone fragmentation , it is extremely difficult to obtain abundant product ions ( other than Na + ) from ( M + Na ) + brevetoxin precursor ions in low-energy collision-induced dissociation ( CID ) MS/MS experiments .
	manualset3
264798	7	424249	15	NULL	NULL	NULL	NULL	( M + Na ) + brevetoxin precursor ions 	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the ionic charge tends to remain localized on the sodium atom and because at least two bonds must be broken in order to produce polycyclic backbone fragmentation , it is extremely difficult to obtain abundant product ions ( other than Na + ) from ( M + Na ) + brevetoxin precursor ions in low-energy collision-induced dissociation ( CID ) MS/MS experiments .
	manualset3
264799	8	424249	15	NULL	NULL	NULL	NULL	low-energy collision-induced dissociation ( CID ) MS/MS experiments	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the ionic charge tends to remain localized on the sodium atom and because at least two bonds must be broken in order to produce polycyclic backbone fragmentation , it is extremely difficult to obtain abundant product ions ( other than Na + ) from ( M + Na ) + brevetoxin precursor ions in low-energy collision-induced dissociation ( CID ) MS/MS experiments .
	manualset3
264800	1	424250	15	NULL	NULL	NULL	NULL	nursing staff 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the nursing staff of the Gynecology Day Surgery Unit at the Royal Victoria Hospital believes there is a need for patient-monitoring after discharge and CLSCs do not offer services for this generally healthy clientele , they developed , with the head nurse and the assistant head nurse , a post-operative telephone follow-up program .
	manualset3
264801	2	424250	15	NULL	NULL	NULL	NULL	Gynecology Day Surgery Unit 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the nursing staff of the Gynecology Day Surgery Unit at the Royal Victoria Hospital believes there is a need for patient-monitoring after discharge and CLSCs do not offer services for this generally healthy clientele , they developed , with the head nurse and the assistant head nurse , a post-operative telephone follow-up program .
	manualset3
264802	3	424250	15	NULL	NULL	NULL	NULL	Royal Victoria Hospital	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the nursing staff of the Gynecology Day Surgery Unit at the Royal Victoria Hospital believes there is a need for patient-monitoring after discharge and CLSCs do not offer services for this generally healthy clientele , they developed , with the head nurse and the assistant head nurse , a post-operative telephone follow-up program .
	manualset3
264803	4	424250	15	NULL	NULL	NULL	NULL	patient-monitoring	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the nursing staff of the Gynecology Day Surgery Unit at the Royal Victoria Hospital believes there is a need for patient-monitoring after discharge and CLSCs do not offer services for this generally healthy clientele , they developed , with the head nurse and the assistant head nurse , a post-operative telephone follow-up program .
	manualset3
264804	5	424250	15	NULL	NULL	NULL	NULL	discharge	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the nursing staff of the Gynecology Day Surgery Unit at the Royal Victoria Hospital believes there is a need for patient-monitoring after discharge and CLSCs do not offer services for this generally healthy clientele , they developed , with the head nurse and the assistant head nurse , a post-operative telephone follow-up program .
	manualset3
264805	6	424250	15	NULL	NULL	NULL	NULL	CLSCs	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the nursing staff of the Gynecology Day Surgery Unit at the Royal Victoria Hospital believes there is a need for patient-monitoring after discharge and CLSCs do not offer services for this generally healthy clientele , they developed , with the head nurse and the assistant head nurse , a post-operative telephone follow-up program .
	manualset3
264806	7	424250	15	NULL	NULL	NULL	NULL	services	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the nursing staff of the Gynecology Day Surgery Unit at the Royal Victoria Hospital believes there is a need for patient-monitoring after discharge and CLSCs do not offer services for this generally healthy clientele , they developed , with the head nurse and the assistant head nurse , a post-operative telephone follow-up program .
	manualset3
264807	8	424250	15	NULL	NULL	NULL	NULL	generally healthy clientele	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the nursing staff of the Gynecology Day Surgery Unit at the Royal Victoria Hospital believes there is a need for patient-monitoring after discharge and CLSCs do not offer services for this generally healthy clientele , they developed , with the head nurse and the assistant head nurse , a post-operative telephone follow-up program .
	manualset3
264808	9	424250	15	NULL	NULL	NULL	NULL	head nurse	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the nursing staff of the Gynecology Day Surgery Unit at the Royal Victoria Hospital believes there is a need for patient-monitoring after discharge and CLSCs do not offer services for this generally healthy clientele , they developed , with the head nurse and the assistant head nurse , a post-operative telephone follow-up program .
	manualset3
264809	10	424250	15	NULL	NULL	NULL	NULL	assistant head nurse	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the nursing staff of the Gynecology Day Surgery Unit at the Royal Victoria Hospital believes there is a need for patient-monitoring after discharge and CLSCs do not offer services for this generally healthy clientele , they developed , with the head nurse and the assistant head nurse , a post-operative telephone follow-up program .
	manualset3
264810	11	424250	15	NULL	NULL	NULL	NULL	post-operative telephone follow-up program	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the nursing staff of the Gynecology Day Surgery Unit at the Royal Victoria Hospital believes there is a need for patient-monitoring after discharge and CLSCs do not offer services for this generally healthy clientele , they developed , with the head nurse and the assistant head nurse , a post-operative telephone follow-up program .
	manualset3
264812	1	424251	15	NULL	NULL	NULL	NULL	organism	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the organism can not be cultivated on artificial media the diagnosis of the aetiological agent Clostridium piliforme is rather difficult and is based on the identification of typical gross lesions and histological demonstration of the characteristic intracellular bacteria at the periphery of the necrotic foci .
	manualset3
264813	2	424251	15	NULL	NULL	NULL	NULL	artificial media	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the organism can not be cultivated on artificial media the diagnosis of the aetiological agent Clostridium piliforme is rather difficult and is based on the identification of typical gross lesions and histological demonstration of the characteristic intracellular bacteria at the periphery of the necrotic foci .
	manualset3
264814	3	424251	15	NULL	NULL	NULL	NULL	diagnosis 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the organism can not be cultivated on artificial media the diagnosis of the aetiological agent Clostridium piliforme is rather difficult and is based on the identification of typical gross lesions and histological demonstration of the characteristic intracellular bacteria at the periphery of the necrotic foci .
	manualset3
264815	4	424251	15	NULL	NULL	NULL	NULL	aetiological agent	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the organism can not be cultivated on artificial media the diagnosis of the aetiological agent Clostridium piliforme is rather difficult and is based on the identification of typical gross lesions and histological demonstration of the characteristic intracellular bacteria at the periphery of the necrotic foci .
	manualset3
264816	5	424251	15	NULL	NULL	NULL	NULL	Clostridium piliforme 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the organism can not be cultivated on artificial media the diagnosis of the aetiological agent Clostridium piliforme is rather difficult and is based on the identification of typical gross lesions and histological demonstration of the characteristic intracellular bacteria at the periphery of the necrotic foci .
	manualset3
264817	6	424251	15	NULL	NULL	NULL	NULL	identification	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the organism can not be cultivated on artificial media the diagnosis of the aetiological agent Clostridium piliforme is rather difficult and is based on the identification of typical gross lesions and histological demonstration of the characteristic intracellular bacteria at the periphery of the necrotic foci .
	manualset3
264818	7	424251	15	NULL	NULL	NULL	NULL	typical gross lesions 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the organism can not be cultivated on artificial media the diagnosis of the aetiological agent Clostridium piliforme is rather difficult and is based on the identification of typical gross lesions and histological demonstration of the characteristic intracellular bacteria at the periphery of the necrotic foci .
	manualset3
264819	8	424251	15	NULL	NULL	NULL	NULL	histological demonstration	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the organism can not be cultivated on artificial media the diagnosis of the aetiological agent Clostridium piliforme is rather difficult and is based on the identification of typical gross lesions and histological demonstration of the characteristic intracellular bacteria at the periphery of the necrotic foci .
	manualset3
264820	9	424251	15	NULL	NULL	NULL	NULL	intracellular bacteria	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the organism can not be cultivated on artificial media the diagnosis of the aetiological agent Clostridium piliforme is rather difficult and is based on the identification of typical gross lesions and histological demonstration of the characteristic intracellular bacteria at the periphery of the necrotic foci .
	manualset3
264821	10	424251	15	NULL	NULL	NULL	NULL	periphery of the necrotic foci 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the organism can not be cultivated on artificial media the diagnosis of the aetiological agent Clostridium piliforme is rather difficult and is based on the identification of typical gross lesions and histological demonstration of the characteristic intracellular bacteria at the periphery of the necrotic foci .
	manualset3
264822	1	424252	15	NULL	NULL	NULL	NULL	parents	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the parents were consanguineous , we performed homozygosity mapping to identify homozygous regions containing candidate genes such as NDUFA2 on chromosome 5 .
	manualset3
264823	2	424252	15	NULL	NULL	NULL	NULL	homozygosity mapping	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the parents were consanguineous , we performed homozygosity mapping to identify homozygous regions containing candidate genes such as NDUFA2 on chromosome 5 .
	manualset3
264824	3	424252	15	NULL	NULL	NULL	NULL	homozygous regions	Chromosome												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the parents were consanguineous , we performed homozygosity mapping to identify homozygous regions containing candidate genes such as NDUFA2 on chromosome 5 .
	manualset3
264825	4	424252	15	NULL	NULL	NULL	NULL	candidate genes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the parents were consanguineous , we performed homozygosity mapping to identify homozygous regions containing candidate genes such as NDUFA2 on chromosome 5 .
	manualset3
264826	5	424252	15	NULL	NULL	NULL	NULL	NDUFA2	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the parents were consanguineous , we performed homozygosity mapping to identify homozygous regions containing candidate genes such as NDUFA2 on chromosome 5 .
	manualset3
264827	6	424252	15	NULL	NULL	NULL	NULL	chromosome 5	Chromosome												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because the parents were consanguineous , we performed homozygosity mapping to identify homozygous regions containing candidate genes such as NDUFA2 on chromosome 5 .
	manualset3
264828	1	424253	15	NULL	NULL	NULL	NULL	differences 	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because there are important differences between the culture , research base , and decision-making processes of clinicians and managers , the ideas of evidence-based practice , while relevant , need to be translated for management rather than simply transferred .
	manualset3
264829	2	424253	15	NULL	NULL	NULL	NULL	culture	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because there are important differences between the culture , research base , and decision-making processes of clinicians and managers , the ideas of evidence-based practice , while relevant , need to be translated for management rather than simply transferred .
	manualset3
264830	3	424253	15	NULL	NULL	NULL	NULL	research base	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because there are important differences between the culture , research base , and decision-making processes of clinicians and managers , the ideas of evidence-based practice , while relevant , need to be translated for management rather than simply transferred .
	manualset3
264831	4	424253	15	NULL	NULL	NULL	NULL	decision-making processes	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because there are important differences between the culture , research base , and decision-making processes of clinicians and managers , the ideas of evidence-based practice , while relevant , need to be translated for management rather than simply transferred .
	manualset3
264832	5	424253	15	NULL	NULL	NULL	NULL	clinicians	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because there are important differences between the culture , research base , and decision-making processes of clinicians and managers , the ideas of evidence-based practice , while relevant , need to be translated for management rather than simply transferred .
	manualset3
264833	6	424253	15	NULL	NULL	NULL	NULL	managers	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because there are important differences between the culture , research base , and decision-making processes of clinicians and managers , the ideas of evidence-based practice , while relevant , need to be translated for management rather than simply transferred .
	manualset3
264834	7	424253	15	NULL	NULL	NULL	NULL	ideas	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because there are important differences between the culture , research base , and decision-making processes of clinicians and managers , the ideas of evidence-based practice , while relevant , need to be translated for management rather than simply transferred .
	manualset3
264835	8	424253	15	NULL	NULL	NULL	NULL	evidence-based practice	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because there are important differences between the culture , research base , and decision-making processes of clinicians and managers , the ideas of evidence-based practice , while relevant , need to be translated for management rather than simply transferred .
	manualset3
264836	9	424253	15	NULL	NULL	NULL	NULL	management	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because there are important differences between the culture , research base , and decision-making processes of clinicians and managers , the ideas of evidence-based practice , while relevant , need to be translated for management rather than simply transferred .
	manualset3
264837	1	424254	15	NULL	NULL	NULL	NULL	rabbits 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because these rabbits were cholesterol-clamped , the antiatherogenic effect was not mediated via plasma cholesterol lowering .
	manualset3
264838	2	424254	15	NULL	NULL	NULL	NULL	cholesterol-clamped	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because these rabbits were cholesterol-clamped , the antiatherogenic effect was not mediated via plasma cholesterol lowering .
	manualset3
264839	3	424254	15	NULL	NULL	NULL	NULL	antiatherogenic effect	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because these rabbits were cholesterol-clamped , the antiatherogenic effect was not mediated via plasma cholesterol lowering .
	manualset3
264840	4	424254	15	NULL	NULL	NULL	NULL	plasma cholesterol	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because these rabbits were cholesterol-clamped , the antiatherogenic effect was not mediated via plasma cholesterol lowering .
	manualset3
264841	1	424255	15	NULL	NULL	NULL	NULL	disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because this disease showed distinctive clinical manifestations and characteristic histopathological features , we believe it is a distinct entity and should be distinguished from other types of vasculitis .
	manualset3
264842	2	424255	15	NULL	NULL	NULL	NULL	clinical manifestations 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because this disease showed distinctive clinical manifestations and characteristic histopathological features , we believe it is a distinct entity and should be distinguished from other types of vasculitis .
	manualset3
264843	3	424255	15	NULL	NULL	NULL	NULL	histopathological features	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because this disease showed distinctive clinical manifestations and characteristic histopathological features , we believe it is a distinct entity and should be distinguished from other types of vasculitis .
	manualset3
264844	4	424255	15	NULL	NULL	NULL	NULL	entity	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because this disease showed distinctive clinical manifestations and characteristic histopathological features , we believe it is a distinct entity and should be distinguished from other types of vasculitis .
	manualset3
264845	5	424255	15	NULL	NULL	NULL	NULL	types of vasculitis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because this disease showed distinctive clinical manifestations and characteristic histopathological features , we believe it is a distinct entity and should be distinguished from other types of vasculitis .
	manualset3
264846	1	424256	15	NULL	NULL	NULL	NULL	preparation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because this preparation separates the predominantly direct effects of UPEEP on the ipsilateral lung from its indirect effects on the contralateral lung , it is well suited to studies of direct pulmonary vascular effects of airway pressure changes in an intact closed-chest preparation with reactive pulmonary vasculature .
	manualset3
264847	2	424256	15	NULL	NULL	NULL	NULL	direct effects	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because this preparation separates the predominantly direct effects of UPEEP on the ipsilateral lung from its indirect effects on the contralateral lung , it is well suited to studies of direct pulmonary vascular effects of airway pressure changes in an intact closed-chest preparation with reactive pulmonary vasculature .
	manualset3
264848	3	424256	15	NULL	NULL	NULL	NULL	UPEEP	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because this preparation separates the predominantly direct effects of UPEEP on the ipsilateral lung from its indirect effects on the contralateral lung , it is well suited to studies of direct pulmonary vascular effects of airway pressure changes in an intact closed-chest preparation with reactive pulmonary vasculature .
	manualset3
264849	4	424256	15	NULL	NULL	NULL	NULL	ipsilateral lung	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because this preparation separates the predominantly direct effects of UPEEP on the ipsilateral lung from its indirect effects on the contralateral lung , it is well suited to studies of direct pulmonary vascular effects of airway pressure changes in an intact closed-chest preparation with reactive pulmonary vasculature .
	manualset3
264850	5	424256	15	NULL	NULL	NULL	NULL	indirect effects	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because this preparation separates the predominantly direct effects of UPEEP on the ipsilateral lung from its indirect effects on the contralateral lung , it is well suited to studies of direct pulmonary vascular effects of airway pressure changes in an intact closed-chest preparation with reactive pulmonary vasculature .
	manualset3
264851	6	424256	15	NULL	NULL	NULL	NULL	contralateral lung	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because this preparation separates the predominantly direct effects of UPEEP on the ipsilateral lung from its indirect effects on the contralateral lung , it is well suited to studies of direct pulmonary vascular effects of airway pressure changes in an intact closed-chest preparation with reactive pulmonary vasculature .
	manualset3
264852	7	424256	15	NULL	NULL	NULL	NULL	studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because this preparation separates the predominantly direct effects of UPEEP on the ipsilateral lung from its indirect effects on the contralateral lung , it is well suited to studies of direct pulmonary vascular effects of airway pressure changes in an intact closed-chest preparation with reactive pulmonary vasculature .
	manualset3
264853	8	424256	15	NULL	NULL	NULL	NULL	direct pulmonary vascular effects 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because this preparation separates the predominantly direct effects of UPEEP on the ipsilateral lung from its indirect effects on the contralateral lung , it is well suited to studies of direct pulmonary vascular effects of airway pressure changes in an intact closed-chest preparation with reactive pulmonary vasculature .
	manualset3
264854	9	424256	15	NULL	NULL	NULL	NULL	airway pressure changes	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because this preparation separates the predominantly direct effects of UPEEP on the ipsilateral lung from its indirect effects on the contralateral lung , it is well suited to studies of direct pulmonary vascular effects of airway pressure changes in an intact closed-chest preparation with reactive pulmonary vasculature .
	manualset3
264855	10	424256	15	NULL	NULL	NULL	NULL	intact closed-chest preparation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because this preparation separates the predominantly direct effects of UPEEP on the ipsilateral lung from its indirect effects on the contralateral lung , it is well suited to studies of direct pulmonary vascular effects of airway pressure changes in an intact closed-chest preparation with reactive pulmonary vasculature .
	manualset3
264856	11	424256	15	NULL	NULL	NULL	NULL	reactive pulmonary vasculature	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Because this preparation separates the predominantly direct effects of UPEEP on the ipsilateral lung from its indirect effects on the contralateral lung , it is well suited to studies of direct pulmonary vascular effects of airway pressure changes in an intact closed-chest preparation with reactive pulmonary vasculature .
	manualset3
264857	1	424257	15	NULL	NULL	NULL	NULL	FAMILIAL HERPETIC DISEASE	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( FAMILIAL HERPETIC DISEASE ) .
	manualset3
264858	1	424258	15	NULL	NULL	NULL	NULL	BeefX	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BeefX had greater birth weight calves ( P = 0.01 ) , greater IGF-II ( P & lt ; 0.001 ) , increased ratios of IGF-I : total IGFBP ( P = 0.008 ) and IGF-II : total IGFBP ( P & lt ; 0.001 ) , and reduced total IGFBP compared with CBX ( P = 0.02 ) .
	manualset3
264859	2	424258	15	NULL	NULL	NULL	NULL	birth weight	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BeefX had greater birth weight calves ( P = 0.01 ) , greater IGF-II ( P & lt ; 0.001 ) , increased ratios of IGF-I : total IGFBP ( P = 0.008 ) and IGF-II : total IGFBP ( P & lt ; 0.001 ) , and reduced total IGFBP compared with CBX ( P = 0.02 ) .
	manualset3
264860	3	424258	15	NULL	NULL	NULL	NULL	calves	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BeefX had greater birth weight calves ( P = 0.01 ) , greater IGF-II ( P & lt ; 0.001 ) , increased ratios of IGF-I : total IGFBP ( P = 0.008 ) and IGF-II : total IGFBP ( P & lt ; 0.001 ) , and reduced total IGFBP compared with CBX ( P = 0.02 ) .
	manualset3
264861	4	424258	15	NULL	NULL	NULL	NULL	P = 0.01	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BeefX had greater birth weight calves ( P = 0.01 ) , greater IGF-II ( P & lt ; 0.001 ) , increased ratios of IGF-I : total IGFBP ( P = 0.008 ) and IGF-II : total IGFBP ( P & lt ; 0.001 ) , and reduced total IGFBP compared with CBX ( P = 0.02 ) .
	manualset3
264862	5	424258	15	NULL	NULL	NULL	NULL	IGF-II	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BeefX had greater birth weight calves ( P = 0.01 ) , greater IGF-II ( P & lt ; 0.001 ) , increased ratios of IGF-I : total IGFBP ( P = 0.008 ) and IGF-II : total IGFBP ( P & lt ; 0.001 ) , and reduced total IGFBP compared with CBX ( P = 0.02 ) .
	manualset3
264863	6	424258	15	NULL	NULL	NULL	NULL	P & lt ; 0.001	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BeefX had greater birth weight calves ( P = 0.01 ) , greater IGF-II ( P & lt ; 0.001 ) , increased ratios of IGF-I : total IGFBP ( P = 0.008 ) and IGF-II : total IGFBP ( P & lt ; 0.001 ) , and reduced total IGFBP compared with CBX ( P = 0.02 ) .
	manualset3
264864	7	424258	15	NULL	NULL	NULL	NULL	ratios 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BeefX had greater birth weight calves ( P = 0.01 ) , greater IGF-II ( P & lt ; 0.001 ) , increased ratios of IGF-I : total IGFBP ( P = 0.008 ) and IGF-II : total IGFBP ( P & lt ; 0.001 ) , and reduced total IGFBP compared with CBX ( P = 0.02 ) .
	manualset3
264865	8	424258	15	NULL	NULL	NULL	NULL	IGF-I	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BeefX had greater birth weight calves ( P = 0.01 ) , greater IGF-II ( P & lt ; 0.001 ) , increased ratios of IGF-I : total IGFBP ( P = 0.008 ) and IGF-II : total IGFBP ( P & lt ; 0.001 ) , and reduced total IGFBP compared with CBX ( P = 0.02 ) .
	manualset3
264866	9	424258	15	NULL	NULL	NULL	NULL	IGFBP	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BeefX had greater birth weight calves ( P = 0.01 ) , greater IGF-II ( P & lt ; 0.001 ) , increased ratios of IGF-I : total IGFBP ( P = 0.008 ) and IGF-II : total IGFBP ( P & lt ; 0.001 ) , and reduced total IGFBP compared with CBX ( P = 0.02 ) .
	manualset3
264867	10	424258	15	NULL	NULL	NULL	NULL	P = 0.008	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BeefX had greater birth weight calves ( P = 0.01 ) , greater IGF-II ( P & lt ; 0.001 ) , increased ratios of IGF-I : total IGFBP ( P = 0.008 ) and IGF-II : total IGFBP ( P & lt ; 0.001 ) , and reduced total IGFBP compared with CBX ( P = 0.02 ) .
	manualset3
264868	11	424258	15	NULL	NULL	NULL	NULL	IGF-II	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BeefX had greater birth weight calves ( P = 0.01 ) , greater IGF-II ( P & lt ; 0.001 ) , increased ratios of IGF-I : total IGFBP ( P = 0.008 ) and IGF-II : total IGFBP ( P & lt ; 0.001 ) , and reduced total IGFBP compared with CBX ( P = 0.02 ) .
	manualset3
264869	12	424258	15	NULL	NULL	NULL	NULL	total IGFBP ( P & lt ; 0.001 )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BeefX had greater birth weight calves ( P = 0.01 ) , greater IGF-II ( P & lt ; 0.001 ) , increased ratios of IGF-I : total IGFBP ( P = 0.008 ) and IGF-II : total IGFBP ( P & lt ; 0.001 ) , and reduced total IGFBP compared with CBX ( P = 0.02 ) .
	manualset3
264870	13	424258	15	NULL	NULL	NULL	NULL	total IGFBP	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BeefX had greater birth weight calves ( P = 0.01 ) , greater IGF-II ( P & lt ; 0.001 ) , increased ratios of IGF-I : total IGFBP ( P = 0.008 ) and IGF-II : total IGFBP ( P & lt ; 0.001 ) , and reduced total IGFBP compared with CBX ( P = 0.02 ) .
	manualset3
264871	14	424258	15	NULL	NULL	NULL	NULL	CBX ( P = 0.02 )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	BeefX had greater birth weight calves ( P = 0.01 ) , greater IGF-II ( P & lt ; 0.001 ) , increased ratios of IGF-I : total IGFBP ( P = 0.008 ) and IGF-II : total IGFBP ( P & lt ; 0.001 ) , and reduced total IGFBP compared with CBX ( P = 0.02 ) .
	manualset3
264872	1	424259	15	NULL	NULL	NULL	NULL	anaesthesia	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before anaesthesia , 50 % of all patients had symptoms of moderate to severe hunger , while 44 % of patients had symptoms of moderate to severe thirst .
	manualset3
264873	2	424259	15	NULL	NULL	NULL	NULL	50 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before anaesthesia , 50 % of all patients had symptoms of moderate to severe hunger , while 44 % of patients had symptoms of moderate to severe thirst .
	manualset3
264874	3	424259	15	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before anaesthesia , 50 % of all patients had symptoms of moderate to severe hunger , while 44 % of patients had symptoms of moderate to severe thirst .
	manualset3
264875	4	424259	15	NULL	NULL	NULL	NULL	symptoms 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before anaesthesia , 50 % of all patients had symptoms of moderate to severe hunger , while 44 % of patients had symptoms of moderate to severe thirst .
	manualset3
264876	5	424259	15	NULL	NULL	NULL	NULL	severe hunger	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before anaesthesia , 50 % of all patients had symptoms of moderate to severe hunger , while 44 % of patients had symptoms of moderate to severe thirst .
	manualset3
264877	6	424259	15	NULL	NULL	NULL	NULL	44 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before anaesthesia , 50 % of all patients had symptoms of moderate to severe hunger , while 44 % of patients had symptoms of moderate to severe thirst .
	manualset3
264878	7	424259	15	NULL	NULL	NULL	NULL	patients 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before anaesthesia , 50 % of all patients had symptoms of moderate to severe hunger , while 44 % of patients had symptoms of moderate to severe thirst .
	manualset3
264879	8	424259	15	NULL	NULL	NULL	NULL	symptoms 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before anaesthesia , 50 % of all patients had symptoms of moderate to severe hunger , while 44 % of patients had symptoms of moderate to severe thirst .
	manualset3
264880	9	424259	15	NULL	NULL	NULL	NULL	severe thirst	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before anaesthesia , 50 % of all patients had symptoms of moderate to severe hunger , while 44 % of patients had symptoms of moderate to severe thirst .
	manualset3
264936	1	424260	15	NULL	NULL	NULL	NULL	exposure scenario	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before and after each exposure scenario , volunteers were submitted to a battery of sensory tests ( visual and olfactory ) , neuropsychological tests ( reaction time , attention , memory , psychomotor function ) , and self-evaluation questionnaires ( mood and symptoms ) in a test-retest design .
	manualset3
264937	2	424260	15	NULL	NULL	NULL	NULL	volunteers 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before and after each exposure scenario , volunteers were submitted to a battery of sensory tests ( visual and olfactory ) , neuropsychological tests ( reaction time , attention , memory , psychomotor function ) , and self-evaluation questionnaires ( mood and symptoms ) in a test-retest design .
	manualset3
264939	3	424260	15	NULL	NULL	NULL	NULL	battery of sensory tests 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before and after each exposure scenario , volunteers were submitted to a battery of sensory tests ( visual and olfactory ) , neuropsychological tests ( reaction time , attention , memory , psychomotor function ) , and self-evaluation questionnaires ( mood and symptoms ) in a test-retest design .
	manualset3
264945	4	424260	15	NULL	NULL	NULL	NULL	neuropsychological tests	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before and after each exposure scenario , volunteers were submitted to a battery of sensory tests ( visual and olfactory ) , neuropsychological tests ( reaction time , attention , memory , psychomotor function ) , and self-evaluation questionnaires ( mood and symptoms ) in a test-retest design .
	manualset3
264946	5	424260	15	NULL	NULL	NULL	NULL	reaction time 	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before and after each exposure scenario , volunteers were submitted to a battery of sensory tests ( visual and olfactory ) , neuropsychological tests ( reaction time , attention , memory , psychomotor function ) , and self-evaluation questionnaires ( mood and symptoms ) in a test-retest design .
	manualset3
264947	6	424260	15	NULL	NULL	NULL	NULL	attention	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before and after each exposure scenario , volunteers were submitted to a battery of sensory tests ( visual and olfactory ) , neuropsychological tests ( reaction time , attention , memory , psychomotor function ) , and self-evaluation questionnaires ( mood and symptoms ) in a test-retest design .
	manualset3
264948	7	424260	15	NULL	NULL	NULL	NULL	memory 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before and after each exposure scenario , volunteers were submitted to a battery of sensory tests ( visual and olfactory ) , neuropsychological tests ( reaction time , attention , memory , psychomotor function ) , and self-evaluation questionnaires ( mood and symptoms ) in a test-retest design .
	manualset3
264949	8	424260	15	NULL	NULL	NULL	NULL	psychomotor function 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before and after each exposure scenario , volunteers were submitted to a battery of sensory tests ( visual and olfactory ) , neuropsychological tests ( reaction time , attention , memory , psychomotor function ) , and self-evaluation questionnaires ( mood and symptoms ) in a test-retest design .
	manualset3
264950	9	424260	15	NULL	NULL	NULL	NULL	self-evaluation questionnaires 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before and after each exposure scenario , volunteers were submitted to a battery of sensory tests ( visual and olfactory ) , neuropsychological tests ( reaction time , attention , memory , psychomotor function ) , and self-evaluation questionnaires ( mood and symptoms ) in a test-retest design .
	manualset3
264951	10	424260	15	NULL	NULL	NULL	NULL	 mood	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before and after each exposure scenario , volunteers were submitted to a battery of sensory tests ( visual and olfactory ) , neuropsychological tests ( reaction time , attention , memory , psychomotor function ) , and self-evaluation questionnaires ( mood and symptoms ) in a test-retest design .
	manualset3
264952	11	424260	15	NULL	NULL	NULL	NULL	symptoms	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before and after each exposure scenario , volunteers were submitted to a battery of sensory tests ( visual and olfactory ) , neuropsychological tests ( reaction time , attention , memory , psychomotor function ) , and self-evaluation questionnaires ( mood and symptoms ) in a test-retest design .
	manualset3
264953	12	424260	15	NULL	NULL	NULL	NULL	test-retest design	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before and after each exposure scenario , volunteers were submitted to a battery of sensory tests ( visual and olfactory ) , neuropsychological tests ( reaction time , attention , memory , psychomotor function ) , and self-evaluation questionnaires ( mood and symptoms ) in a test-retest design .
	manualset3
264954	1	424261	15	NULL	NULL	NULL	NULL	inhalation period	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before each inhalation period , participants underwent a training procedure aimed at encouraging them either to mindfully observe ( acceptance context ) or to control symptoms via diaphragmatic breathing ( control context ) .
	manualset3
264955	2	424261	15	NULL	NULL	NULL	NULL	participants 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before each inhalation period , participants underwent a training procedure aimed at encouraging them either to mindfully observe ( acceptance context ) or to control symptoms via diaphragmatic breathing ( control context ) .
	manualset3
264956	3	424261	15	NULL	NULL	NULL	NULL	training procedure	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before each inhalation period , participants underwent a training procedure aimed at encouraging them either to mindfully observe ( acceptance context ) or to control symptoms via diaphragmatic breathing ( control context ) .
	manualset3
264958	4	424261	15	NULL	NULL	NULL	NULL	observe	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before each inhalation period , participants underwent a training procedure aimed at encouraging them either to mindfully observe ( acceptance context ) or to control symptoms via diaphragmatic breathing ( control context ) .
	manualset3
264962	5	424261	15	NULL	NULL	NULL	NULL	acceptance context	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before each inhalation period , participants underwent a training procedure aimed at encouraging them either to mindfully observe ( acceptance context ) or to control symptoms via diaphragmatic breathing ( control context ) .
	manualset3
264963	6	424261	15	NULL	NULL	NULL	NULL	symptoms	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before each inhalation period , participants underwent a training procedure aimed at encouraging them either to mindfully observe ( acceptance context ) or to control symptoms via diaphragmatic breathing ( control context ) .
	manualset3
264964	7	424261	15	NULL	NULL	NULL	NULL	diaphragmatic breathing 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before each inhalation period , participants underwent a training procedure aimed at encouraging them either to mindfully observe ( acceptance context ) or to control symptoms via diaphragmatic breathing ( control context ) .
	manualset3
264967	8	424261	15	NULL	NULL	NULL	NULL	control context	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before each inhalation period , participants underwent a training procedure aimed at encouraging them either to mindfully observe ( acceptance context ) or to control symptoms via diaphragmatic breathing ( control context ) .
	manualset3
264970	1	424262	15	NULL	NULL	NULL	NULL	implantation 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before implantation , in vitro sensor sensitivity was similar to values obtained after explantation ( 0.66 + / - 0.09 vs 1.07 + / - 0.19 nA/mM , n = 9 , p = ns ) .
	manualset3
264972	2	424262	15	NULL	NULL	NULL	NULL	sensor sensitivity	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before implantation , in vitro sensor sensitivity was similar to values obtained after explantation ( 0.66 + / - 0.09 vs 1.07 + / - 0.19 nA/mM , n = 9 , p = ns ) .
	manualset3
264974	3	424262	15	NULL	NULL	NULL	NULL	values 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before implantation , in vitro sensor sensitivity was similar to values obtained after explantation ( 0.66 + / - 0.09 vs 1.07 + / - 0.19 nA/mM , n = 9 , p = ns ) .
	manualset3
264976	4	424262	15	NULL	NULL	NULL	NULL	explantation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before implantation , in vitro sensor sensitivity was similar to values obtained after explantation ( 0.66 + / - 0.09 vs 1.07 + / - 0.19 nA/mM , n = 9 , p = ns ) .
	manualset3
264978	5	424262	15	NULL	NULL	NULL	NULL	0.66 + / - 0.09 vs 1.07 + / - 0.19 nA/mM 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before implantation , in vitro sensor sensitivity was similar to values obtained after explantation ( 0.66 + / - 0.09 vs 1.07 + / - 0.19 nA/mM , n = 9 , p = ns ) .
	manualset3
264980	6	424262	15	NULL	NULL	NULL	NULL	n = 9 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before implantation , in vitro sensor sensitivity was similar to values obtained after explantation ( 0.66 + / - 0.09 vs 1.07 + / - 0.19 nA/mM , n = 9 , p = ns ) .
	manualset3
264981	7	424262	15	NULL	NULL	NULL	NULL	p = ns 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before implantation , in vitro sensor sensitivity was similar to values obtained after explantation ( 0.66 + / - 0.09 vs 1.07 + / - 0.19 nA/mM , n = 9 , p = ns ) .
	manualset3
264982	1	424263	15	NULL	NULL	NULL	NULL	operation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before operation and after anasthesia with 50 mg/kg ketamine and 8 mg/kg xylazine , spinal evoked potentials ( SEP ) were recorded in all rabbits .
	manualset3
264983	2	424263	15	NULL	NULL	NULL	NULL	anasthesia	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before operation and after anasthesia with 50 mg/kg ketamine and 8 mg/kg xylazine , spinal evoked potentials ( SEP ) were recorded in all rabbits .
	manualset3
264984	3	424263	15	NULL	NULL	NULL	NULL	50 mg/kg 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before operation and after anasthesia with 50 mg/kg ketamine and 8 mg/kg xylazine , spinal evoked potentials ( SEP ) were recorded in all rabbits .
	manualset3
264985	4	424263	15	NULL	NULL	NULL	NULL	ketamine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before operation and after anasthesia with 50 mg/kg ketamine and 8 mg/kg xylazine , spinal evoked potentials ( SEP ) were recorded in all rabbits .
	manualset3
264986	5	424263	15	NULL	NULL	NULL	NULL	8 mg/kg	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before operation and after anasthesia with 50 mg/kg ketamine and 8 mg/kg xylazine , spinal evoked potentials ( SEP ) were recorded in all rabbits .
	manualset3
264987	6	424263	15	NULL	NULL	NULL	NULL	xylazine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before operation and after anasthesia with 50 mg/kg ketamine and 8 mg/kg xylazine , spinal evoked potentials ( SEP ) were recorded in all rabbits .
	manualset3
264988	7	424263	15	NULL	NULL	NULL	NULL	spinal evoked potentials ( SEP ) 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before operation and after anasthesia with 50 mg/kg ketamine and 8 mg/kg xylazine , spinal evoked potentials ( SEP ) were recorded in all rabbits .
	manualset3
264989	8	424263	15	NULL	NULL	NULL	NULL	rabbits	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before operation and after anasthesia with 50 mg/kg ketamine and 8 mg/kg xylazine , spinal evoked potentials ( SEP ) were recorded in all rabbits .
	manualset3
264990	1	424264	15	NULL	NULL	NULL	NULL	antidepressant agent	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before prescribing an antidepressant agent , the specific guidelines , side-effect profile , drug-drug interactions and most current indications should always be obtained .
	manualset3
264991	2	424264	15	NULL	NULL	NULL	NULL	specific guidelines	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before prescribing an antidepressant agent , the specific guidelines , side-effect profile , drug-drug interactions and most current indications should always be obtained .
	manualset3
264992	3	424264	15	NULL	NULL	NULL	NULL	side-effect profile	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before prescribing an antidepressant agent , the specific guidelines , side-effect profile , drug-drug interactions and most current indications should always be obtained .
	manualset3
264993	4	424264	15	NULL	NULL	NULL	NULL	drug-drug interactions 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before prescribing an antidepressant agent , the specific guidelines , side-effect profile , drug-drug interactions and most current indications should always be obtained .
	manualset3
264994	5	424264	15	NULL	NULL	NULL	NULL	current indications	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before prescribing an antidepressant agent , the specific guidelines , side-effect profile , drug-drug interactions and most current indications should always be obtained .
	manualset3
264995	1	424265	15	NULL	NULL	NULL	NULL	FIXATION	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( FIXATION OF LONG BONE FRACTURES WITH MODIFIED KLIMOV 'S PLATE ) .
	manualset3
264997	2	424265	15	NULL	NULL	NULL	NULL	LONG BONE FRACTURES 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( FIXATION OF LONG BONE FRACTURES WITH MODIFIED KLIMOV 'S PLATE ) .
	manualset3
264998	3	424265	15	NULL	NULL	NULL	NULL	MODIFIED KLIMOV 'S PLATE	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( FIXATION OF LONG BONE FRACTURES WITH MODIFIED KLIMOV 'S PLATE ) .
	manualset3
264999	1	424266	15	NULL	NULL	NULL	NULL	colitis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before the onset of colitis 3 patients had receive prednisone , associated in 2 of them with immunosuppressive drugs .
	manualset3
265000	2	424266	15	NULL	NULL	NULL	NULL	3 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before the onset of colitis 3 patients had receive prednisone , associated in 2 of them with immunosuppressive drugs .
	manualset3
265001	3	424266	15	NULL	NULL	NULL	NULL	prednisone	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before the onset of colitis 3 patients had receive prednisone , associated in 2 of them with immunosuppressive drugs .
	manualset3
265002	4	424266	15	NULL	NULL	NULL	NULL	2 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before the onset of colitis 3 patients had receive prednisone , associated in 2 of them with immunosuppressive drugs .
	manualset3
265003	5	424266	15	NULL	NULL	NULL	NULL	immunosuppressive drugs 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before the onset of colitis 3 patients had receive prednisone , associated in 2 of them with immunosuppressive drugs .
	manualset3
265004	1	424267	15	NULL	NULL	NULL	NULL	 operation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before the operation primarily the authors confirmed at the patients the presence of menstrual abnormalities in 96.8 % , of infertility in 100 % , of hirsutism I. in 9.7 % , II .
	manualset3
265005	2	424267	15	NULL	NULL	NULL	NULL	authors 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before the operation primarily the authors confirmed at the patients the presence of menstrual abnormalities in 96.8 % , of infertility in 100 % , of hirsutism I. in 9.7 % , II .
	manualset3
265006	3	424267	15	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before the operation primarily the authors confirmed at the patients the presence of menstrual abnormalities in 96.8 % , of infertility in 100 % , of hirsutism I. in 9.7 % , II .
	manualset3
265007	4	424267	15	NULL	NULL	NULL	NULL	presence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before the operation primarily the authors confirmed at the patients the presence of menstrual abnormalities in 96.8 % , of infertility in 100 % , of hirsutism I. in 9.7 % , II .
	manualset3
265008	5	424267	15	NULL	NULL	NULL	NULL	menstrual abnormalities	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before the operation primarily the authors confirmed at the patients the presence of menstrual abnormalities in 96.8 % , of infertility in 100 % , of hirsutism I. in 9.7 % , II .
	manualset3
265009	6	424267	15	NULL	NULL	NULL	NULL	96.8 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before the operation primarily the authors confirmed at the patients the presence of menstrual abnormalities in 96.8 % , of infertility in 100 % , of hirsutism I. in 9.7 % , II .
	manualset3
265010	7	424267	15	NULL	NULL	NULL	NULL	infertility 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before the operation primarily the authors confirmed at the patients the presence of menstrual abnormalities in 96.8 % , of infertility in 100 % , of hirsutism I. in 9.7 % , II .
	manualset3
265011	8	424267	15	NULL	NULL	NULL	NULL	100 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before the operation primarily the authors confirmed at the patients the presence of menstrual abnormalities in 96.8 % , of infertility in 100 % , of hirsutism I. in 9.7 % , II .
	manualset3
265012	9	424267	15	NULL	NULL	NULL	NULL	hirsutism I.	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before the operation primarily the authors confirmed at the patients the presence of menstrual abnormalities in 96.8 % , of infertility in 100 % , of hirsutism I. in 9.7 % , II .
	manualset3
265013	10	424267	15	NULL	NULL	NULL	NULL	9.7 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before the operation primarily the authors confirmed at the patients the presence of menstrual abnormalities in 96.8 % , of infertility in 100 % , of hirsutism I. in 9.7 % , II .
	manualset3
265036	11	424267	15	NULL	NULL	NULL	NULL	 hirsutism II 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before the operation primarily the authors confirmed at the patients the presence of menstrual abnormalities in 96.8 % , of infertility in 100 % , of hirsutism I. in 9.7 % , II .
	manualset3
265041	1	424268	15	NULL	NULL	NULL	NULL	therapy 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before therapy is decided upon it is important to know what the etiology is .
	manualset3
265042	2	424268	15	NULL	NULL	NULL	NULL	etiology 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before therapy is decided upon it is important to know what the etiology is .
	manualset3
265043	1	424269	15	NULL	NULL	NULL	NULL	treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before treatment we found no changes in D2 binding in 10 patients ( in comparison to 10 normal controls ) .
	manualset3
265044	2	424269	15	NULL	NULL	NULL	NULL	 changes	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before treatment we found no changes in D2 binding in 10 patients ( in comparison to 10 normal controls ) .
	manualset3
265045	3	424269	15	NULL	NULL	NULL	NULL	D2 binding	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before treatment we found no changes in D2 binding in 10 patients ( in comparison to 10 normal controls ) .
	manualset3
265046	4	424269	15	NULL	NULL	NULL	NULL	10 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before treatment we found no changes in D2 binding in 10 patients ( in comparison to 10 normal controls ) .
	manualset3
265047	5	424269	15	NULL	NULL	NULL	NULL	10 normal controls	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Before treatment we found no changes in D2 binding in 10 patients ( in comparison to 10 normal controls ) .
	manualset3
265048	1	424270	15	NULL	NULL	NULL	NULL	Beginning in 1970	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Beginning in 1970 , the respective two-breed crosses and the four-breed cross ( Polypay ) were each mated inter se and selected , along with straightbred Rambouillets and Targhees , for lamb production when given two opportunities to lamb/year .
	manualset3
265049	2	424270	15	NULL	NULL	NULL	NULL	two-breed crosses	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Beginning in 1970 , the respective two-breed crosses and the four-breed cross ( Polypay ) were each mated inter se and selected , along with straightbred Rambouillets and Targhees , for lamb production when given two opportunities to lamb/year .
	manualset3
265050	3	424270	15	NULL	NULL	NULL	NULL	four-breed cross 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Beginning in 1970 , the respective two-breed crosses and the four-breed cross ( Polypay ) were each mated inter se and selected , along with straightbred Rambouillets and Targhees , for lamb production when given two opportunities to lamb/year .
	manualset3
265051	4	424270	15	NULL	NULL	NULL	NULL	Polypay 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Beginning in 1970 , the respective two-breed crosses and the four-breed cross ( Polypay ) were each mated inter se and selected , along with straightbred Rambouillets and Targhees , for lamb production when given two opportunities to lamb/year .
	manualset3
265052	5	424270	15	NULL	NULL	NULL	NULL	straightbred Rambouillets	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Beginning in 1970 , the respective two-breed crosses and the four-breed cross ( Polypay ) were each mated inter se and selected , along with straightbred Rambouillets and Targhees , for lamb production when given two opportunities to lamb/year .
	manualset3
265053	6	424270	15	NULL	NULL	NULL	NULL	straightbred Targhees	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Beginning in 1970 , the respective two-breed crosses and the four-breed cross ( Polypay ) were each mated inter se and selected , along with straightbred Rambouillets and Targhees , for lamb production when given two opportunities to lamb/year .
	manualset3
265054	7	424270	15	NULL	NULL	NULL	NULL	lamb production	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Beginning in 1970 , the respective two-breed crosses and the four-breed cross ( Polypay ) were each mated inter se and selected , along with straightbred Rambouillets and Targhees , for lamb production when given two opportunities to lamb/year .
	manualset3
265055	8	424270	15	NULL	NULL	NULL	NULL	two 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Beginning in 1970 , the respective two-breed crosses and the four-breed cross ( Polypay ) were each mated inter se and selected , along with straightbred Rambouillets and Targhees , for lamb production when given two opportunities to lamb/year .
	manualset3
265056	9	424270	15	NULL	NULL	NULL	NULL	opportunities	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Beginning in 1970 , the respective two-breed crosses and the four-breed cross ( Polypay ) were each mated inter se and selected , along with straightbred Rambouillets and Targhees , for lamb production when given two opportunities to lamb/year .
	manualset3
265057	1	424271	15	NULL	NULL	NULL	NULL	Behav Brain Res 2004 ; 155 : 147 -52	Journal												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behav Brain Res 2004 ; 155 : 147 -52 ) , hippocampal lesions cause strong deficits in spatial orientation .
	manualset3
265060	2	424271	15	NULL	NULL	NULL	NULL	hippocampal lesions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behav Brain Res 2004 ; 155 : 147 -52 ) , hippocampal lesions cause strong deficits in spatial orientation .
	manualset3
265061	3	424271	15	NULL	NULL	NULL	NULL	deficits 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behav Brain Res 2004 ; 155 : 147 -52 ) , hippocampal lesions cause strong deficits in spatial orientation .
	manualset3
265062	4	424271	15	NULL	NULL	NULL	NULL	spatial orientation 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behav Brain Res 2004 ; 155 : 147 -52 ) , hippocampal lesions cause strong deficits in spatial orientation .
	manualset3
265063	1	424272	15	NULL	NULL	NULL	NULL	Behavior problems	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavior problems of young girls with fragile X syndrome : factor scores on the Conners ' Parent 's Questionnaire .
	manualset3
265064	2	424272	15	NULL	NULL	NULL	NULL	young girls 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavior problems of young girls with fragile X syndrome : factor scores on the Conners ' Parent 's Questionnaire .
	manualset3
265065	3	424272	15	NULL	NULL	NULL	NULL	fragile X syndrome : factor scores 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavior problems of young girls with fragile X syndrome : factor scores on the Conners ' Parent 's Questionnaire .
	manualset3
265066	4	424272	15	NULL	NULL	NULL	NULL	Conners ' Parent 's Questionnaire 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavior problems of young girls with fragile X syndrome : factor scores on the Conners ' Parent 's Questionnaire .
	manualset3
265067	1	424273	15	NULL	NULL	NULL	NULL	Behavioral responses	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral , hormonal , and morphological responses of free-living male pied flycatchers to estradiol treatment of their mates .
	manualset3
265068	2	424273	15	NULL	NULL	NULL	NULL	hormonal  responses	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral , hormonal , and morphological responses of free-living male pied flycatchers to estradiol treatment of their mates .
	manualset3
265069	3	424273	15	NULL	NULL	NULL	NULL	morphological responses	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral , hormonal , and morphological responses of free-living male pied flycatchers to estradiol treatment of their mates .
	manualset3
265070	4	424273	15	NULL	NULL	NULL	NULL	free-living male pied flycatchers	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral , hormonal , and morphological responses of free-living male pied flycatchers to estradiol treatment of their mates .
	manualset3
265071	5	424273	15	NULL	NULL	NULL	NULL	estradiol treatment 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral , hormonal , and morphological responses of free-living male pied flycatchers to estradiol treatment of their mates .
	manualset3
265072	6	424273	15	NULL	NULL	NULL	NULL	mates	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral , hormonal , and morphological responses of free-living male pied flycatchers to estradiol treatment of their mates .
	manualset3
265073	1	424274	15	NULL	NULL	NULL	NULL	Behavioral correlates	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral correlates in the happy puppet syndrome : a characteristic profile ?
	manualset3
265074	2	424274	15	NULL	NULL	NULL	NULL	happy puppet syndrome	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral correlates in the happy puppet syndrome : a characteristic profile ?
	manualset3
265075	3	424274	15	NULL	NULL	NULL	NULL	characteristic profile 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral correlates in the happy puppet syndrome : a characteristic profile ?
	manualset3
265161	1	424275	15	NULL	NULL	NULL	NULL	family	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( A family of congenital factor XI ( PTA ) deficiency ) .
	manualset3
265163	2	424275	15	NULL	NULL	NULL	NULL	congenital factor XI ( PTA ) deficiency	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( A family of congenital factor XI ( PTA ) deficiency ) .
	manualset3
265164	1	424276	15	NULL	NULL	NULL	NULL	Fall	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Fall in blood pressure caused by spinal anesthesia in cesarean section .
	manualset3
265165	2	424276	15	NULL	NULL	NULL	NULL	blood pressure	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Fall in blood pressure caused by spinal anesthesia in cesarean section .
	manualset3
265166	3	424276	15	NULL	NULL	NULL	NULL	spinal anesthesia	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Fall in blood pressure caused by spinal anesthesia in cesarean section .
	manualset3
265167	4	424276	15	NULL	NULL	NULL	NULL	cesarean section 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Fall in blood pressure caused by spinal anesthesia in cesarean section .
	manualset3
265168	1	424277	15	NULL	NULL	NULL	NULL	Behavioral evidence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral evidence suggests that 5-HT3 receptors interact with mesolimbic dopamine ( DA ) systems and that 5-HT3 antagonists can interfere with the hyperlocomotive effects of amphetamine and cocaine and the rewarding and stimulus effects of morphine , nicotine and ethanol .
	manualset3
265169	2	424277	15	NULL	NULL	NULL	NULL	5-HT3 receptors	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral evidence suggests that 5-HT3 receptors interact with mesolimbic dopamine ( DA ) systems and that 5-HT3 antagonists can interfere with the hyperlocomotive effects of amphetamine and cocaine and the rewarding and stimulus effects of morphine , nicotine and ethanol .
	manualset3
265170	3	424277	15	NULL	NULL	NULL	NULL	mesolimbic dopamine ( DA ) systems	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral evidence suggests that 5-HT3 receptors interact with mesolimbic dopamine ( DA ) systems and that 5-HT3 antagonists can interfere with the hyperlocomotive effects of amphetamine and cocaine and the rewarding and stimulus effects of morphine , nicotine and ethanol .
	manualset3
265171	4	424277	15	NULL	NULL	NULL	NULL	5-HT3 antagonists 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral evidence suggests that 5-HT3 receptors interact with mesolimbic dopamine ( DA ) systems and that 5-HT3 antagonists can interfere with the hyperlocomotive effects of amphetamine and cocaine and the rewarding and stimulus effects of morphine , nicotine and ethanol .
	manualset3
265172	5	424277	15	NULL	NULL	NULL	NULL	hyperlocomotive effects	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral evidence suggests that 5-HT3 receptors interact with mesolimbic dopamine ( DA ) systems and that 5-HT3 antagonists can interfere with the hyperlocomotive effects of amphetamine and cocaine and the rewarding and stimulus effects of morphine , nicotine and ethanol .
	manualset3
265173	6	424277	15	NULL	NULL	NULL	NULL	amphetamine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral evidence suggests that 5-HT3 receptors interact with mesolimbic dopamine ( DA ) systems and that 5-HT3 antagonists can interfere with the hyperlocomotive effects of amphetamine and cocaine and the rewarding and stimulus effects of morphine , nicotine and ethanol .
	manualset3
265174	7	424277	15	NULL	NULL	NULL	NULL	cocaine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral evidence suggests that 5-HT3 receptors interact with mesolimbic dopamine ( DA ) systems and that 5-HT3 antagonists can interfere with the hyperlocomotive effects of amphetamine and cocaine and the rewarding and stimulus effects of morphine , nicotine and ethanol .
	manualset3
265175	8	424277	15	NULL	NULL	NULL	NULL	stimulus effects 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral evidence suggests that 5-HT3 receptors interact with mesolimbic dopamine ( DA ) systems and that 5-HT3 antagonists can interfere with the hyperlocomotive effects of amphetamine and cocaine and the rewarding and stimulus effects of morphine , nicotine and ethanol .
	manualset3
265176	9	424277	15	NULL	NULL	NULL	NULL	morphine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral evidence suggests that 5-HT3 receptors interact with mesolimbic dopamine ( DA ) systems and that 5-HT3 antagonists can interfere with the hyperlocomotive effects of amphetamine and cocaine and the rewarding and stimulus effects of morphine , nicotine and ethanol .
	manualset3
265177	10	424277	15	NULL	NULL	NULL	NULL	nicotine 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral evidence suggests that 5-HT3 receptors interact with mesolimbic dopamine ( DA ) systems and that 5-HT3 antagonists can interfere with the hyperlocomotive effects of amphetamine and cocaine and the rewarding and stimulus effects of morphine , nicotine and ethanol .
	manualset3
265178	11	424277	15	NULL	NULL	NULL	NULL	ethanol	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral evidence suggests that 5-HT3 receptors interact with mesolimbic dopamine ( DA ) systems and that 5-HT3 antagonists can interfere with the hyperlocomotive effects of amphetamine and cocaine and the rewarding and stimulus effects of morphine , nicotine and ethanol .
	manualset3
265186	1	424278	15	NULL	NULL	NULL	NULL	pre-test data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral pre-test data revealed that while listening to Japanese short-duration ( 100 % : reference ) , long-duration ( 180 % ) , and other in-between duration-synthesized types , healthy native speakers of Japanese failed to clearly categorize 140-124 % durations as either short or long words , while categorizing 108-116 % durations as short words and 148-172 % durations as long .
	manualset3
265188	2	424278	15	NULL	NULL	NULL	NULL	Japanese short-duration	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral pre-test data revealed that while listening to Japanese short-duration ( 100 % : reference ) , long-duration ( 180 % ) , and other in-between duration-synthesized types , healthy native speakers of Japanese failed to clearly categorize 140-124 % durations as either short or long words , while categorizing 108-116 % durations as short words and 148-172 % durations as long .
	manualset3
265189	3	424278	15	NULL	NULL	NULL	NULL	100 % : reference 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral pre-test data revealed that while listening to Japanese short-duration ( 100 % : reference ) , long-duration ( 180 % ) , and other in-between duration-synthesized types , healthy native speakers of Japanese failed to clearly categorize 140-124 % durations as either short or long words , while categorizing 108-116 % durations as short words and 148-172 % durations as long .
	manualset3
265190	4	424278	15	NULL	NULL	NULL	NULL	long-duration 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral pre-test data revealed that while listening to Japanese short-duration ( 100 % : reference ) , long-duration ( 180 % ) , and other in-between duration-synthesized types , healthy native speakers of Japanese failed to clearly categorize 140-124 % durations as either short or long words , while categorizing 108-116 % durations as short words and 148-172 % durations as long .
	manualset3
265191	5	424278	15	NULL	NULL	NULL	NULL	180 % 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral pre-test data revealed that while listening to Japanese short-duration ( 100 % : reference ) , long-duration ( 180 % ) , and other in-between duration-synthesized types , healthy native speakers of Japanese failed to clearly categorize 140-124 % durations as either short or long words , while categorizing 108-116 % durations as short words and 148-172 % durations as long .
	manualset3
265192	6	424278	15	NULL	NULL	NULL	NULL	duration-synthesized types 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral pre-test data revealed that while listening to Japanese short-duration ( 100 % : reference ) , long-duration ( 180 % ) , and other in-between duration-synthesized types , healthy native speakers of Japanese failed to clearly categorize 140-124 % durations as either short or long words , while categorizing 108-116 % durations as short words and 148-172 % durations as long .
	manualset3
265193	7	424278	15	NULL	NULL	NULL	NULL	healthy native speakers	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral pre-test data revealed that while listening to Japanese short-duration ( 100 % : reference ) , long-duration ( 180 % ) , and other in-between duration-synthesized types , healthy native speakers of Japanese failed to clearly categorize 140-124 % durations as either short or long words , while categorizing 108-116 % durations as short words and 148-172 % durations as long .
	manualset3
265194	8	424278	15	NULL	NULL	NULL	NULL	Japanese	Language												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral pre-test data revealed that while listening to Japanese short-duration ( 100 % : reference ) , long-duration ( 180 % ) , and other in-between duration-synthesized types , healthy native speakers of Japanese failed to clearly categorize 140-124 % durations as either short or long words , while categorizing 108-116 % durations as short words and 148-172 % durations as long .
	manualset3
265195	9	424278	15	NULL	NULL	NULL	NULL	categorize	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral pre-test data revealed that while listening to Japanese short-duration ( 100 % : reference ) , long-duration ( 180 % ) , and other in-between duration-synthesized types , healthy native speakers of Japanese failed to clearly categorize 140-124 % durations as either short or long words , while categorizing 108-116 % durations as short words and 148-172 % durations as long .
	manualset3
265196	10	424278	15	NULL	NULL	NULL	NULL	140-124 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral pre-test data revealed that while listening to Japanese short-duration ( 100 % : reference ) , long-duration ( 180 % ) , and other in-between duration-synthesized types , healthy native speakers of Japanese failed to clearly categorize 140-124 % durations as either short or long words , while categorizing 108-116 % durations as short words and 148-172 % durations as long .
	manualset3
265197	11	424278	15	NULL	NULL	NULL	NULL	durations 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral pre-test data revealed that while listening to Japanese short-duration ( 100 % : reference ) , long-duration ( 180 % ) , and other in-between duration-synthesized types , healthy native speakers of Japanese failed to clearly categorize 140-124 % durations as either short or long words , while categorizing 108-116 % durations as short words and 148-172 % durations as long .
	manualset3
265198	12	424278	15	NULL	NULL	NULL	NULL	short words	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral pre-test data revealed that while listening to Japanese short-duration ( 100 % : reference ) , long-duration ( 180 % ) , and other in-between duration-synthesized types , healthy native speakers of Japanese failed to clearly categorize 140-124 % durations as either short or long words , while categorizing 108-116 % durations as short words and 148-172 % durations as long .
	manualset3
265199	13	424278	15	NULL	NULL	NULL	NULL	long words	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral pre-test data revealed that while listening to Japanese short-duration ( 100 % : reference ) , long-duration ( 180 % ) , and other in-between duration-synthesized types , healthy native speakers of Japanese failed to clearly categorize 140-124 % durations as either short or long words , while categorizing 108-116 % durations as short words and 148-172 % durations as long .
	manualset3
265200	14	424278	15	NULL	NULL	NULL	NULL	108-116 % 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral pre-test data revealed that while listening to Japanese short-duration ( 100 % : reference ) , long-duration ( 180 % ) , and other in-between duration-synthesized types , healthy native speakers of Japanese failed to clearly categorize 140-124 % durations as either short or long words , while categorizing 108-116 % durations as short words and 148-172 % durations as long .
	manualset3
265201	15	424278	15	NULL	NULL	NULL	NULL	durations 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral pre-test data revealed that while listening to Japanese short-duration ( 100 % : reference ) , long-duration ( 180 % ) , and other in-between duration-synthesized types , healthy native speakers of Japanese failed to clearly categorize 140-124 % durations as either short or long words , while categorizing 108-116 % durations as short words and 148-172 % durations as long .
	manualset3
265202	16	424278	15	NULL	NULL	NULL	NULL	short words	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral pre-test data revealed that while listening to Japanese short-duration ( 100 % : reference ) , long-duration ( 180 % ) , and other in-between duration-synthesized types , healthy native speakers of Japanese failed to clearly categorize 140-124 % durations as either short or long words , while categorizing 108-116 % durations as short words and 148-172 % durations as long .
	manualset3
265203	17	424278	15	NULL	NULL	NULL	NULL	148-172 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral pre-test data revealed that while listening to Japanese short-duration ( 100 % : reference ) , long-duration ( 180 % ) , and other in-between duration-synthesized types , healthy native speakers of Japanese failed to clearly categorize 140-124 % durations as either short or long words , while categorizing 108-116 % durations as short words and 148-172 % durations as long .
	manualset3
265204	18	424278	15	NULL	NULL	NULL	NULL	durations 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral pre-test data revealed that while listening to Japanese short-duration ( 100 % : reference ) , long-duration ( 180 % ) , and other in-between duration-synthesized types , healthy native speakers of Japanese failed to clearly categorize 140-124 % durations as either short or long words , while categorizing 108-116 % durations as short words and 148-172 % durations as long .
	manualset3
265205	1	424279	15	NULL	NULL	NULL	NULL	Behavioral studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral studies demonstrated further that the cell-permeable cGMP analog 8-bromoadenosine-cGMP reverses the inhibitory effects of the alpha ( 1 ) - adrenoceptor antagonist prazosin on lordosis behavior in E ( 2 ) - and P-treated female rats .
	manualset3
265206	2	424279	15	NULL	NULL	NULL	NULL	cell-permeable cGMP analog 	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral studies demonstrated further that the cell-permeable cGMP analog 8-bromoadenosine-cGMP reverses the inhibitory effects of the alpha ( 1 ) - adrenoceptor antagonist prazosin on lordosis behavior in E ( 2 ) - and P-treated female rats .
	manualset3
265207	3	424279	15	NULL	NULL	NULL	NULL	8-bromoadenosine-cGMP	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral studies demonstrated further that the cell-permeable cGMP analog 8-bromoadenosine-cGMP reverses the inhibitory effects of the alpha ( 1 ) - adrenoceptor antagonist prazosin on lordosis behavior in E ( 2 ) - and P-treated female rats .
	manualset3
265208	4	424279	15	NULL	NULL	NULL	NULL	inhibitory effects 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral studies demonstrated further that the cell-permeable cGMP analog 8-bromoadenosine-cGMP reverses the inhibitory effects of the alpha ( 1 ) - adrenoceptor antagonist prazosin on lordosis behavior in E ( 2 ) - and P-treated female rats .
	manualset3
265209	5	424279	15	NULL	NULL	NULL	NULL	alpha ( 1 ) - adrenoceptor antagonist 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral studies demonstrated further that the cell-permeable cGMP analog 8-bromoadenosine-cGMP reverses the inhibitory effects of the alpha ( 1 ) - adrenoceptor antagonist prazosin on lordosis behavior in E ( 2 ) - and P-treated female rats .
	manualset3
265210	6	424279	15	NULL	NULL	NULL	NULL	prazosin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral studies demonstrated further that the cell-permeable cGMP analog 8-bromoadenosine-cGMP reverses the inhibitory effects of the alpha ( 1 ) - adrenoceptor antagonist prazosin on lordosis behavior in E ( 2 ) - and P-treated female rats .
	manualset3
265211	7	424279	15	NULL	NULL	NULL	NULL	lordosis behavior	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral studies demonstrated further that the cell-permeable cGMP analog 8-bromoadenosine-cGMP reverses the inhibitory effects of the alpha ( 1 ) - adrenoceptor antagonist prazosin on lordosis behavior in E ( 2 ) - and P-treated female rats .
	manualset3
265212	8	424279	15	NULL	NULL	NULL	NULL	E ( 2 ) treated female rats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral studies demonstrated further that the cell-permeable cGMP analog 8-bromoadenosine-cGMP reverses the inhibitory effects of the alpha ( 1 ) - adrenoceptor antagonist prazosin on lordosis behavior in E ( 2 ) - and P-treated female rats .
	manualset3
265213	9	424279	15	NULL	NULL	NULL	NULL	P-treated female rats 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral studies demonstrated further that the cell-permeable cGMP analog 8-bromoadenosine-cGMP reverses the inhibitory effects of the alpha ( 1 ) - adrenoceptor antagonist prazosin on lordosis behavior in E ( 2 ) - and P-treated female rats .
	manualset3
265214	1	424280	15	NULL	NULL	NULL	NULL	Behavioral testing	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral testing started 2 weeks following irradiation .
	manualset3
265215	2	424280	15	NULL	NULL	NULL	NULL	2 weeks	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral testing started 2 weeks following irradiation .
	manualset3
265216	3	424280	15	NULL	NULL	NULL	NULL	irradiation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behavioral testing started 2 weeks following irradiation .
	manualset3
265217	1	424281	15	NULL	NULL	NULL	NULL	Behaviorally augmented tolerance	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behaviorally augmented tolerance during chronic cholinesterase reduction by paraoxon .
	manualset3
265218	2	424281	15	NULL	NULL	NULL	NULL	chronic cholinesterase reduction 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behaviorally augmented tolerance during chronic cholinesterase reduction by paraoxon .
	manualset3
265219	3	424281	15	NULL	NULL	NULL	NULL	paraoxon	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behaviorally augmented tolerance during chronic cholinesterase reduction by paraoxon .
	manualset3
265220	1	424282	15	NULL	NULL	NULL	NULL	Behaviours	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behaviours associated with affective disorders ranging along the affective spectrum from depression to dysphoric mania may be particularly amenable to valproic acid .
	manualset3
265221	2	424282	15	NULL	NULL	NULL	NULL	affective disorders	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behaviours associated with affective disorders ranging along the affective spectrum from depression to dysphoric mania may be particularly amenable to valproic acid .
	manualset3
265222	3	424282	15	NULL	NULL	NULL	NULL	affective spectrum	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behaviours associated with affective disorders ranging along the affective spectrum from depression to dysphoric mania may be particularly amenable to valproic acid .
	manualset3
265223	4	424282	15	NULL	NULL	NULL	NULL	depression	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behaviours associated with affective disorders ranging along the affective spectrum from depression to dysphoric mania may be particularly amenable to valproic acid .
	manualset3
265224	5	424282	15	NULL	NULL	NULL	NULL	dysphoric mania	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behaviours associated with affective disorders ranging along the affective spectrum from depression to dysphoric mania may be particularly amenable to valproic acid .
	manualset3
265225	6	424282	15	NULL	NULL	NULL	NULL	valproic acid 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behaviours associated with affective disorders ranging along the affective spectrum from depression to dysphoric mania may be particularly amenable to valproic acid .
	manualset3
265226	1	424283	15	NULL	NULL	NULL	NULL	Behcet 's disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behcet 's disease is a multisystem disorder and classified as `` vasculitic syndrome with a wide variety of clinical manifestations . ''
	manualset3
265227	2	424283	15	NULL	NULL	NULL	NULL	multisystem disorder 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behcet 's disease is a multisystem disorder and classified as `` vasculitic syndrome with a wide variety of clinical manifestations . ''
	manualset3
265228	3	424283	15	NULL	NULL	NULL	NULL	vasculitic syndrome	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behcet 's disease is a multisystem disorder and classified as `` vasculitic syndrome with a wide variety of clinical manifestations . ''
	manualset3
265229	4	424283	15	NULL	NULL	NULL	NULL	variety 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behcet 's disease is a multisystem disorder and classified as `` vasculitic syndrome with a wide variety of clinical manifestations . ''
	manualset3
265230	5	424283	15	NULL	NULL	NULL	NULL	clinical manifestations	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Behcet 's disease is a multisystem disorder and classified as `` vasculitic syndrome with a wide variety of clinical manifestations . ''
	manualset3
265231	1	424284	15	NULL	NULL	NULL	NULL	single dose	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Being administered in a single dose of 30 mg/kg , 1 h after irradiation , PCL prevented hypertension development in an early post-irradiated period ( 9 days ) .
	manualset3
265232	2	424284	15	NULL	NULL	NULL	NULL	30 mg/kg	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Being administered in a single dose of 30 mg/kg , 1 h after irradiation , PCL prevented hypertension development in an early post-irradiated period ( 9 days ) .
	manualset3
265233	3	424284	15	NULL	NULL	NULL	NULL	1 h 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Being administered in a single dose of 30 mg/kg , 1 h after irradiation , PCL prevented hypertension development in an early post-irradiated period ( 9 days ) .
	manualset3
265234	4	424284	15	NULL	NULL	NULL	NULL	 irradiation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Being administered in a single dose of 30 mg/kg , 1 h after irradiation , PCL prevented hypertension development in an early post-irradiated period ( 9 days ) .
	manualset3
265235	5	424284	15	NULL	NULL	NULL	NULL	PCL	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Being administered in a single dose of 30 mg/kg , 1 h after irradiation , PCL prevented hypertension development in an early post-irradiated period ( 9 days ) .
	manualset3
265236	6	424284	15	NULL	NULL	NULL	NULL	hypertension development	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Being administered in a single dose of 30 mg/kg , 1 h after irradiation , PCL prevented hypertension development in an early post-irradiated period ( 9 days ) .
	manualset3
265237	7	424284	15	NULL	NULL	NULL	NULL	early post-irradiated period	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Being administered in a single dose of 30 mg/kg , 1 h after irradiation , PCL prevented hypertension development in an early post-irradiated period ( 9 days ) .
	manualset3
265238	8	424284	15	NULL	NULL	NULL	NULL	 9 days	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Being administered in a single dose of 30 mg/kg , 1 h after irradiation , PCL prevented hypertension development in an early post-irradiated period ( 9 days ) .
	manualset3
265239	1	424285	15	NULL	NULL	NULL	NULL	 zeolites	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Being amphoteric , zeolites are partly soluble in acid or alkaline media , but within the physiological pH range the solubility is generally low .
	manualset3
265240	2	424285	15	NULL	NULL	NULL	NULL	acid media 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Being amphoteric , zeolites are partly soluble in acid or alkaline media , but within the physiological pH range the solubility is generally low .
	manualset3
265241	3	424285	15	NULL	NULL	NULL	NULL	alkaline media 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Being amphoteric , zeolites are partly soluble in acid or alkaline media , but within the physiological pH range the solubility is generally low .
	manualset3
265242	4	424285	15	NULL	NULL	NULL	NULL	physiological pH range	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Being amphoteric , zeolites are partly soluble in acid or alkaline media , but within the physiological pH range the solubility is generally low .
	manualset3
265243	5	424285	15	NULL	NULL	NULL	NULL	solubility	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Being amphoteric , zeolites are partly soluble in acid or alkaline media , but within the physiological pH range the solubility is generally low .
	manualset3
265252	1	424286	15	NULL	NULL	NULL	NULL	compensation point	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Below the compensation point , two successive field-induced phase transitions and the reversal of the net magnetization of the iron sublattices in the intermediate phase were observed .
	manualset3
265253	2	424286	15	NULL	NULL	NULL	NULL	two	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Below the compensation point , two successive field-induced phase transitions and the reversal of the net magnetization of the iron sublattices in the intermediate phase were observed .
	manualset3
265254	3	424286	15	NULL	NULL	NULL	NULL	field-induced phase transitions	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Below the compensation point , two successive field-induced phase transitions and the reversal of the net magnetization of the iron sublattices in the intermediate phase were observed .
	manualset3
265255	4	424286	15	NULL	NULL	NULL	NULL	reversal 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Below the compensation point , two successive field-induced phase transitions and the reversal of the net magnetization of the iron sublattices in the intermediate phase were observed .
	manualset3
265256	5	424286	15	NULL	NULL	NULL	NULL	net magnetization	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Below the compensation point , two successive field-induced phase transitions and the reversal of the net magnetization of the iron sublattices in the intermediate phase were observed .
	manualset3
265257	6	424286	15	NULL	NULL	NULL	NULL	iron sublattices	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Below the compensation point , two successive field-induced phase transitions and the reversal of the net magnetization of the iron sublattices in the intermediate phase were observed .
	manualset3
265258	7	424286	15	NULL	NULL	NULL	NULL	intermediate phase 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Below the compensation point , two successive field-induced phase transitions and the reversal of the net magnetization of the iron sublattices in the intermediate phase were observed .
	manualset3
265264	1	424287	15	NULL	NULL	NULL	NULL	critical Zn application rate	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Below the critical Zn application rate ( 50 mg kg ( -1 ) ) , Zn uptake was enhanced while above this level Zn translocation to the shoots decreased .
	manualset3
265265	2	424287	15	NULL	NULL	NULL	NULL	50 mg kg ( -1 )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Below the critical Zn application rate ( 50 mg kg ( -1 ) ) , Zn uptake was enhanced while above this level Zn translocation to the shoots decreased .
	manualset3
265267	3	424287	15	NULL	NULL	NULL	NULL	 Zn uptake	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Below the critical Zn application rate ( 50 mg kg ( -1 ) ) , Zn uptake was enhanced while above this level Zn translocation to the shoots decreased .
	manualset3
265269	4	424287	15	NULL	NULL	NULL	NULL	level	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Below the critical Zn application rate ( 50 mg kg ( -1 ) ) , Zn uptake was enhanced while above this level Zn translocation to the shoots decreased .
	manualset3
265271	5	424287	15	NULL	NULL	NULL	NULL	Zn translocation 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Below the critical Zn application rate ( 50 mg kg ( -1 ) ) , Zn uptake was enhanced while above this level Zn translocation to the shoots decreased .
	manualset3
265272	6	424287	15	NULL	NULL	NULL	NULL	shoots	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Below the critical Zn application rate ( 50 mg kg ( -1 ) ) , Zn uptake was enhanced while above this level Zn translocation to the shoots decreased .
	manualset3
265273	1	424288	15	NULL	NULL	NULL	NULL	tc	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Below tc , one observes gel-phase powder patterns which indicate that the bacterial toxin is unable to form such small structures with ordered dipalmitoylglycerophosphocholine phospholipids .
	manualset3
265274	2	424288	15	NULL	NULL	NULL	NULL	gel-phase powder patterns 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Below tc , one observes gel-phase powder patterns which indicate that the bacterial toxin is unable to form such small structures with ordered dipalmitoylglycerophosphocholine phospholipids .
	manualset3
265275	3	424288	15	NULL	NULL	NULL	NULL	bacterial toxin	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Below tc , one observes gel-phase powder patterns which indicate that the bacterial toxin is unable to form such small structures with ordered dipalmitoylglycerophosphocholine phospholipids .
	manualset3
265276	4	424288	15	NULL	NULL	NULL	NULL	small structures 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Below tc , one observes gel-phase powder patterns which indicate that the bacterial toxin is unable to form such small structures with ordered dipalmitoylglycerophosphocholine phospholipids .
	manualset3
265277	5	424288	15	NULL	NULL	NULL	NULL	dipalmitoylglycerophosphocholine phospholipids 	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Below tc , one observes gel-phase powder patterns which indicate that the bacterial toxin is unable to form such small structures with ordered dipalmitoylglycerophosphocholine phospholipids .
	manualset3
265278	1	424289	15	NULL	NULL	NULL	NULL	Benefits	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Benefits of non-invasive ventilation after extubation in the postoperative period of heart surgery .
	manualset3
265279	2	424289	15	NULL	NULL	NULL	NULL	non-invasive ventilation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Benefits of non-invasive ventilation after extubation in the postoperative period of heart surgery .
	manualset3
265280	3	424289	15	NULL	NULL	NULL	NULL	extubation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Benefits of non-invasive ventilation after extubation in the postoperative period of heart surgery .
	manualset3
265281	4	424289	15	NULL	NULL	NULL	NULL	postoperative period	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Benefits of non-invasive ventilation after extubation in the postoperative period of heart surgery .
	manualset3
265282	5	424289	15	NULL	NULL	NULL	NULL	 heart surgery	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Benefits of non-invasive ventilation after extubation in the postoperative period of heart surgery .
	manualset3
265283	1	424290	15	NULL	NULL	NULL	NULL	Benign small bowel tumors 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Benign small bowel tumors are rare .
	manualset3
265285	1	424291	15	NULL	NULL	NULL	NULL	Benthic animal counts	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Benthic animal counts revealed a lack of biodiversity , with relatively low levels of small tubificid oligochaetes ( generally & lt ; 3000/m ( 2 ) ) in surficial sediments .
	manualset3
265287	2	424291	15	NULL	NULL	NULL	NULL	lack of biodiversity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Benthic animal counts revealed a lack of biodiversity , with relatively low levels of small tubificid oligochaetes ( generally & lt ; 3000/m ( 2 ) ) in surficial sediments .
	manualset3
265289	3	424291	15	NULL	NULL	NULL	NULL	low levels	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Benthic animal counts revealed a lack of biodiversity , with relatively low levels of small tubificid oligochaetes ( generally & lt ; 3000/m ( 2 ) ) in surficial sediments .
	manualset3
265290	4	424291	15	NULL	NULL	NULL	NULL	small tubificid oligochaetes	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Benthic animal counts revealed a lack of biodiversity , with relatively low levels of small tubificid oligochaetes ( generally & lt ; 3000/m ( 2 ) ) in surficial sediments .
	manualset3
265291	5	424291	15	NULL	NULL	NULL	NULL	generally & lt ; 3000/m ( 2 ) ) 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Benthic animal counts revealed a lack of biodiversity , with relatively low levels of small tubificid oligochaetes ( generally & lt ; 3000/m ( 2 ) ) in surficial sediments .
	manualset3
265292	6	424291	15	NULL	NULL	NULL	NULL	surficial sediments	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Benthic animal counts revealed a lack of biodiversity , with relatively low levels of small tubificid oligochaetes ( generally & lt ; 3000/m ( 2 ) ) in surficial sediments .
	manualset3
265293	1	424292	15	NULL	NULL	NULL	NULL	Favism	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Favism and anemia caused by sensitivity to primaquine ) .
	manualset3
265294	2	424292	15	NULL	NULL	NULL	NULL	anemia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Favism and anemia caused by sensitivity to primaquine ) .
	manualset3
265295	3	424292	15	NULL	NULL	NULL	NULL	sensitivity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Favism and anemia caused by sensitivity to primaquine ) .
	manualset3
265296	4	424292	15	NULL	NULL	NULL	NULL	primaquine 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Favism and anemia caused by sensitivity to primaquine ) .
	manualset3
265297	1	424293	15	NULL	NULL	NULL	NULL	Benzoflavone activators	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Benzoflavone activators of the cystic fibrosis transmembrane conductance regulator : towards a pharmacophore model for the nucleotide-binding domain .
	manualset3
265298	2	424293	15	NULL	NULL	NULL	NULL	cystic fibrosis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Benzoflavone activators of the cystic fibrosis transmembrane conductance regulator : towards a pharmacophore model for the nucleotide-binding domain .
	manualset3
265299	3	424293	15	NULL	NULL	NULL	NULL	transmembrane conductance regulator	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Benzoflavone activators of the cystic fibrosis transmembrane conductance regulator : towards a pharmacophore model for the nucleotide-binding domain .
	manualset3
265300	4	424293	15	NULL	NULL	NULL	NULL	pharmacophore model	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Benzoflavone activators of the cystic fibrosis transmembrane conductance regulator : towards a pharmacophore model for the nucleotide-binding domain .
	manualset3
265301	5	424293	15	NULL	NULL	NULL	NULL	nucleotide-binding domain	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Benzoflavone activators of the cystic fibrosis transmembrane conductance regulator : towards a pharmacophore model for the nucleotide-binding domain .
	manualset3
265302	1	424294	15	NULL	NULL	NULL	NULL	Benzoyl-coenzyme A	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Benzoyl-coenzyme A and salicoyl-coenzyme A were the preferred starter substrates .
	manualset3
265303	2	424294	15	NULL	NULL	NULL	NULL	salicoyl-coenzyme A	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Benzoyl-coenzyme A and salicoyl-coenzyme A were the preferred starter substrates .
	manualset3
265304	3	424294	15	NULL	NULL	NULL	NULL	starter substrates	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Benzoyl-coenzyme A and salicoyl-coenzyme A were the preferred starter substrates .
	manualset3
265305	1	424295	15	NULL	NULL	NULL	NULL	Bernard-Soulier syndrome	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bernard-Soulier syndrome : an inherited platelet disorder .
	manualset3
265306	2	424295	15	NULL	NULL	NULL	NULL	inherited platelet disorder	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bernard-Soulier syndrome : an inherited platelet disorder .
	manualset3
265307	1	424296	15	NULL	NULL	NULL	NULL	acute hypobaric hypoxia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides , acute hypobaric hypoxia interfered in maternal behavior of females of the FO and F1 generations .
	manualset3
265308	2	424296	15	NULL	NULL	NULL	NULL	maternal behavior	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides , acute hypobaric hypoxia interfered in maternal behavior of females of the FO and F1 generations .
	manualset3
265309	3	424296	15	NULL	NULL	NULL	NULL	females	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides , acute hypobaric hypoxia interfered in maternal behavior of females of the FO and F1 generations .
	manualset3
265310	4	424296	15	NULL	NULL	NULL	NULL	FO generations	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides , acute hypobaric hypoxia interfered in maternal behavior of females of the FO and F1 generations .
	manualset3
265311	5	424296	15	NULL	NULL	NULL	NULL	F1 generations 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides , acute hypobaric hypoxia interfered in maternal behavior of females of the FO and F1 generations .
	manualset3
265312	1	424297	15	NULL	NULL	NULL	NULL	moderate group	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides , in the moderate group , a CBF rebound in vein was found in the post-rewarming phase .
	manualset3
265313	2	424297	15	NULL	NULL	NULL	NULL	CBF	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides , in the moderate group , a CBF rebound in vein was found in the post-rewarming phase .
	manualset3
265314	3	424297	15	NULL	NULL	NULL	NULL	vein	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides , in the moderate group , a CBF rebound in vein was found in the post-rewarming phase .
	manualset3
265315	4	424297	15	NULL	NULL	NULL	NULL	post-rewarming phase 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides , in the moderate group , a CBF rebound in vein was found in the post-rewarming phase .
	manualset3
265316	1	424298	15	NULL	NULL	NULL	NULL	essential role	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides its essential and well established role as a component of the cytoskeleton , actin is also present in the cell nucleus , where it has been linked to many processes that control gene expression .
	manualset3
265317	2	424298	15	NULL	NULL	NULL	NULL	well established role 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides its essential and well established role as a component of the cytoskeleton , actin is also present in the cell nucleus , where it has been linked to many processes that control gene expression .
	manualset3
265318	3	424298	15	NULL	NULL	NULL	NULL	component of the cytoskeleton 	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides its essential and well established role as a component of the cytoskeleton , actin is also present in the cell nucleus , where it has been linked to many processes that control gene expression .
	manualset3
265319	4	424298	15	NULL	NULL	NULL	NULL	actin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides its essential and well established role as a component of the cytoskeleton , actin is also present in the cell nucleus , where it has been linked to many processes that control gene expression .
	manualset3
265320	5	424298	15	NULL	NULL	NULL	NULL	cell nucleus	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides its essential and well established role as a component of the cytoskeleton , actin is also present in the cell nucleus , where it has been linked to many processes that control gene expression .
	manualset3
265321	6	424298	15	NULL	NULL	NULL	NULL	processes	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides its essential and well established role as a component of the cytoskeleton , actin is also present in the cell nucleus , where it has been linked to many processes that control gene expression .
	manualset3
265322	7	424298	15	NULL	NULL	NULL	NULL	gene expression 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides its essential and well established role as a component of the cytoskeleton , actin is also present in the cell nucleus , where it has been linked to many processes that control gene expression .
	manualset3
265323	1	424299	15	NULL	NULL	NULL	NULL	lymphocutaneous forms	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides the lymphocutaneous and fixed forms , other presentations , such as disseminated cutaneous and mucosal involvement , as well as for the first time , erythema nodosum and erythema multiforme have been reported associated with sporotrichosis .
	manualset3
265324	2	424299	15	NULL	NULL	NULL	NULL	fixed forms	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides the lymphocutaneous and fixed forms , other presentations , such as disseminated cutaneous and mucosal involvement , as well as for the first time , erythema nodosum and erythema multiforme have been reported associated with sporotrichosis .
	manualset3
265325	3	424299	15	NULL	NULL	NULL	NULL	presentations	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides the lymphocutaneous and fixed forms , other presentations , such as disseminated cutaneous and mucosal involvement , as well as for the first time , erythema nodosum and erythema multiforme have been reported associated with sporotrichosis .
	manualset3
265326	4	424299	15	NULL	NULL	NULL	NULL	cutaneous involvement	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides the lymphocutaneous and fixed forms , other presentations , such as disseminated cutaneous and mucosal involvement , as well as for the first time , erythema nodosum and erythema multiforme have been reported associated with sporotrichosis .
	manualset3
265327	5	424299	15	NULL	NULL	NULL	NULL	mucosal involvement	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides the lymphocutaneous and fixed forms , other presentations , such as disseminated cutaneous and mucosal involvement , as well as for the first time , erythema nodosum and erythema multiforme have been reported associated with sporotrichosis .
	manualset3
265328	6	424299	15	NULL	NULL	NULL	NULL	time	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides the lymphocutaneous and fixed forms , other presentations , such as disseminated cutaneous and mucosal involvement , as well as for the first time , erythema nodosum and erythema multiforme have been reported associated with sporotrichosis .
	manualset3
265329	7	424299	15	NULL	NULL	NULL	NULL	erythema nodosum 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides the lymphocutaneous and fixed forms , other presentations , such as disseminated cutaneous and mucosal involvement , as well as for the first time , erythema nodosum and erythema multiforme have been reported associated with sporotrichosis .
	manualset3
265330	8	424299	15	NULL	NULL	NULL	NULL	erythema multiforme 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides the lymphocutaneous and fixed forms , other presentations , such as disseminated cutaneous and mucosal involvement , as well as for the first time , erythema nodosum and erythema multiforme have been reported associated with sporotrichosis .
	manualset3
265331	9	424299	15	NULL	NULL	NULL	NULL	sporotrichosis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides the lymphocutaneous and fixed forms , other presentations , such as disseminated cutaneous and mucosal involvement , as well as for the first time , erythema nodosum and erythema multiforme have been reported associated with sporotrichosis .
	manualset3
265332	1	424300	15	NULL	NULL	NULL	NULL	Features of the circulation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Features of the circulation of the fundus oculi in patients with cerebral arteriovenous aneurysms and arteriosinus anastomoses ) .
	manualset3
265333	2	424300	15	NULL	NULL	NULL	NULL	fundus oculi	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Features of the circulation of the fundus oculi in patients with cerebral arteriovenous aneurysms and arteriosinus anastomoses ) .
	manualset3
265334	3	424300	15	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Features of the circulation of the fundus oculi in patients with cerebral arteriovenous aneurysms and arteriosinus anastomoses ) .
	manualset3
265335	4	424300	15	NULL	NULL	NULL	NULL	cerebral arteriovenous aneurysms 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Features of the circulation of the fundus oculi in patients with cerebral arteriovenous aneurysms and arteriosinus anastomoses ) .
	manualset3
265336	5	424300	15	NULL	NULL	NULL	NULL	arteriosinus anastomoses	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Features of the circulation of the fundus oculi in patients with cerebral arteriovenous aneurysms and arteriosinus anastomoses ) .
	manualset3
265337	1	424301	15	NULL	NULL	NULL	NULL	two	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides the two bacterial strains used in the fermented milk , two other lactic acid bacteria , belonging to another genus and unable to induce an immune system response , as well as a strain of Propionibacterium , of which the immune modulating capacity is known , were used in this work .
	manualset3
265338	2	424301	15	NULL	NULL	NULL	NULL	bacterial strains 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides the two bacterial strains used in the fermented milk , two other lactic acid bacteria , belonging to another genus and unable to induce an immune system response , as well as a strain of Propionibacterium , of which the immune modulating capacity is known , were used in this work .
	manualset3
265339	3	424301	15	NULL	NULL	NULL	NULL	fermented milk	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides the two bacterial strains used in the fermented milk , two other lactic acid bacteria , belonging to another genus and unable to induce an immune system response , as well as a strain of Propionibacterium , of which the immune modulating capacity is known , were used in this work .
	manualset3
265340	4	424301	15	NULL	NULL	NULL	NULL	two	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides the two bacterial strains used in the fermented milk , two other lactic acid bacteria , belonging to another genus and unable to induce an immune system response , as well as a strain of Propionibacterium , of which the immune modulating capacity is known , were used in this work .
	manualset3
265341	5	424301	15	NULL	NULL	NULL	NULL	lactic acid bacteria	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides the two bacterial strains used in the fermented milk , two other lactic acid bacteria , belonging to another genus and unable to induce an immune system response , as well as a strain of Propionibacterium , of which the immune modulating capacity is known , were used in this work .
	manualset3
265342	6	424301	15	NULL	NULL	NULL	NULL	genus	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides the two bacterial strains used in the fermented milk , two other lactic acid bacteria , belonging to another genus and unable to induce an immune system response , as well as a strain of Propionibacterium , of which the immune modulating capacity is known , were used in this work .
	manualset3
265343	7	424301	15	NULL	NULL	NULL	NULL	immune system response	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides the two bacterial strains used in the fermented milk , two other lactic acid bacteria , belonging to another genus and unable to induce an immune system response , as well as a strain of Propionibacterium , of which the immune modulating capacity is known , were used in this work .
	manualset3
265344	8	424301	15	NULL	NULL	NULL	NULL	strain of Propionibacterium 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides the two bacterial strains used in the fermented milk , two other lactic acid bacteria , belonging to another genus and unable to induce an immune system response , as well as a strain of Propionibacterium , of which the immune modulating capacity is known , were used in this work .
	manualset3
265345	9	424301	15	NULL	NULL	NULL	NULL	immune modulating capacity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides the two bacterial strains used in the fermented milk , two other lactic acid bacteria , belonging to another genus and unable to induce an immune system response , as well as a strain of Propionibacterium , of which the immune modulating capacity is known , were used in this work .
	manualset3
265346	10	424301	15	NULL	NULL	NULL	NULL	work	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Besides the two bacterial strains used in the fermented milk , two other lactic acid bacteria , belonging to another genus and unable to induce an immune system response , as well as a strain of Propionibacterium , of which the immune modulating capacity is known , were used in this work .
	manualset3
265347	1	424302	15	NULL	NULL	NULL	NULL	mouth care practices 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Best mouth care practices included evidence-based and consensus-based practices as published primarily by the American Dental Association and supported by both published nursing research and review articles specific to mouth care and published dental research and review articles specific to mouth care .
	manualset3
265348	2	424302	15	NULL	NULL	NULL	NULL	evidence-based practices	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Best mouth care practices included evidence-based and consensus-based practices as published primarily by the American Dental Association and supported by both published nursing research and review articles specific to mouth care and published dental research and review articles specific to mouth care .
	manualset3
265349	3	424302	15	NULL	NULL	NULL	NULL	consensus-based practices 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Best mouth care practices included evidence-based and consensus-based practices as published primarily by the American Dental Association and supported by both published nursing research and review articles specific to mouth care and published dental research and review articles specific to mouth care .
	manualset3
265350	4	424302	15	NULL	NULL	NULL	NULL	American Dental Association	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Best mouth care practices included evidence-based and consensus-based practices as published primarily by the American Dental Association and supported by both published nursing research and review articles specific to mouth care and published dental research and review articles specific to mouth care .
	manualset3
265351	5	424302	15	NULL	NULL	NULL	NULL	published nursing research	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Best mouth care practices included evidence-based and consensus-based practices as published primarily by the American Dental Association and supported by both published nursing research and review articles specific to mouth care and published dental research and review articles specific to mouth care .
	manualset3
265352	6	424302	15	NULL	NULL	NULL	NULL	review articles	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Best mouth care practices included evidence-based and consensus-based practices as published primarily by the American Dental Association and supported by both published nursing research and review articles specific to mouth care and published dental research and review articles specific to mouth care .
	manualset3
265353	7	424302	15	NULL	NULL	NULL	NULL	mouth care	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Best mouth care practices included evidence-based and consensus-based practices as published primarily by the American Dental Association and supported by both published nursing research and review articles specific to mouth care and published dental research and review articles specific to mouth care .
	manualset3
265354	8	424302	15	NULL	NULL	NULL	NULL	published dental research 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Best mouth care practices included evidence-based and consensus-based practices as published primarily by the American Dental Association and supported by both published nursing research and review articles specific to mouth care and published dental research and review articles specific to mouth care .
	manualset3
265355	9	424302	15	NULL	NULL	NULL	NULL	review articles	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Best mouth care practices included evidence-based and consensus-based practices as published primarily by the American Dental Association and supported by both published nursing research and review articles specific to mouth care and published dental research and review articles specific to mouth care .
	manualset3
265356	10	424302	15	NULL	NULL	NULL	NULL	mouth care	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Best mouth care practices included evidence-based and consensus-based practices as published primarily by the American Dental Association and supported by both published nursing research and review articles specific to mouth care and published dental research and review articles specific to mouth care .
	manualset3
265357	1	424303	15	NULL	NULL	NULL	NULL	Beta2-integrin clustering	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Beta2-integrin clustering on activation is a key event in leukocyte adhesion to the endothelium during the inflammatory response .
	manualset3
265358	2	424303	15	NULL	NULL	NULL	NULL	activation 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Beta2-integrin clustering on activation is a key event in leukocyte adhesion to the endothelium during the inflammatory response .
	manualset3
265359	3	424303	15	NULL	NULL	NULL	NULL	 key event	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Beta2-integrin clustering on activation is a key event in leukocyte adhesion to the endothelium during the inflammatory response .
	manualset3
265360	4	424303	15	NULL	NULL	NULL	NULL	leukocyte adhesion	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Beta2-integrin clustering on activation is a key event in leukocyte adhesion to the endothelium during the inflammatory response .
	manualset3
265361	5	424303	15	NULL	NULL	NULL	NULL	endothelium 	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Beta2-integrin clustering on activation is a key event in leukocyte adhesion to the endothelium during the inflammatory response .
	manualset3
265362	6	424303	15	NULL	NULL	NULL	NULL	inflammatory response	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Beta2-integrin clustering on activation is a key event in leukocyte adhesion to the endothelium during the inflammatory response .
	manualset3
265363	1	424304	15	NULL	NULL	NULL	NULL	Betaretroviruses	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Betaretroviruses of sheep include two exogenous viruses , Jaagsiekte sheep retrovirus ( JSRV ) and enzootic nasal tumor virus ( ENTV ) , and a group of endogenous viruses known as enJSRVs .
	manualset3
265364	2	424304	15	NULL	NULL	NULL	NULL	sheep 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Betaretroviruses of sheep include two exogenous viruses , Jaagsiekte sheep retrovirus ( JSRV ) and enzootic nasal tumor virus ( ENTV ) , and a group of endogenous viruses known as enJSRVs .
	manualset3
265365	3	424304	15	NULL	NULL	NULL	NULL	two	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Betaretroviruses of sheep include two exogenous viruses , Jaagsiekte sheep retrovirus ( JSRV ) and enzootic nasal tumor virus ( ENTV ) , and a group of endogenous viruses known as enJSRVs .
	manualset3
265366	4	424304	15	NULL	NULL	NULL	NULL	exogenous viruses	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Betaretroviruses of sheep include two exogenous viruses , Jaagsiekte sheep retrovirus ( JSRV ) and enzootic nasal tumor virus ( ENTV ) , and a group of endogenous viruses known as enJSRVs .
	manualset3
265367	5	424304	15	NULL	NULL	NULL	NULL	Jaagsiekte sheep retrovirus ( JSRV )	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Betaretroviruses of sheep include two exogenous viruses , Jaagsiekte sheep retrovirus ( JSRV ) and enzootic nasal tumor virus ( ENTV ) , and a group of endogenous viruses known as enJSRVs .
	manualset3
265368	6	424304	15	NULL	NULL	NULL	NULL	enzootic nasal tumor virus ( ENTV )	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Betaretroviruses of sheep include two exogenous viruses , Jaagsiekte sheep retrovirus ( JSRV ) and enzootic nasal tumor virus ( ENTV ) , and a group of endogenous viruses known as enJSRVs .
	manualset3
265369	7	424304	15	NULL	NULL	NULL	NULL	group of endogenous viruses	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Betaretroviruses of sheep include two exogenous viruses , Jaagsiekte sheep retrovirus ( JSRV ) and enzootic nasal tumor virus ( ENTV ) , and a group of endogenous viruses known as enJSRVs .
	manualset3
265370	8	424304	15	NULL	NULL	NULL	NULL	enJSRVs	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Betaretroviruses of sheep include two exogenous viruses , Jaagsiekte sheep retrovirus ( JSRV ) and enzootic nasal tumor virus ( ENTV ) , and a group of endogenous viruses known as enJSRVs .
	manualset3
265371	1	424305	15	NULL	NULL	NULL	NULL	Better communication	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Better communication among producers , catch-and-fill crews , and others associated with the egg industry , as well as more complete records of dates , sources , and persons involved with pullet placements , are recommended .
	manualset3
265372	2	424305	15	NULL	NULL	NULL	NULL	producers	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Better communication among producers , catch-and-fill crews , and others associated with the egg industry , as well as more complete records of dates , sources , and persons involved with pullet placements , are recommended .
	manualset3
265373	3	424305	15	NULL	NULL	NULL	NULL	catch-and-fill crews	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Better communication among producers , catch-and-fill crews , and others associated with the egg industry , as well as more complete records of dates , sources , and persons involved with pullet placements , are recommended .
	manualset3
265374	4	424305	15	NULL	NULL	NULL	NULL	others 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Better communication among producers , catch-and-fill crews , and others associated with the egg industry , as well as more complete records of dates , sources , and persons involved with pullet placements , are recommended .
	manualset3
265375	5	424305	15	NULL	NULL	NULL	NULL	egg industry	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Better communication among producers , catch-and-fill crews , and others associated with the egg industry , as well as more complete records of dates , sources , and persons involved with pullet placements , are recommended .
	manualset3
265376	6	424305	15	NULL	NULL	NULL	NULL	records of dates	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Better communication among producers , catch-and-fill crews , and others associated with the egg industry , as well as more complete records of dates , sources , and persons involved with pullet placements , are recommended .
	manualset3
265377	7	424305	15	NULL	NULL	NULL	NULL	sources	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Better communication among producers , catch-and-fill crews , and others associated with the egg industry , as well as more complete records of dates , sources , and persons involved with pullet placements , are recommended .
	manualset3
265378	8	424305	15	NULL	NULL	NULL	NULL	persons 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Better communication among producers , catch-and-fill crews , and others associated with the egg industry , as well as more complete records of dates , sources , and persons involved with pullet placements , are recommended .
	manualset3
265379	9	424305	15	NULL	NULL	NULL	NULL	pullet placements 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Better communication among producers , catch-and-fill crews , and others associated with the egg industry , as well as more complete records of dates , sources , and persons involved with pullet placements , are recommended .
	manualset3
265404	1	424306	15	NULL	NULL	NULL	NULL	Field studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Field studies on different control schemes for hookworm infection ) .
	manualset3
265405	2	424306	15	NULL	NULL	NULL	NULL	control schemes	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Field studies on different control schemes for hookworm infection ) .
	manualset3
265406	3	424306	15	NULL	NULL	NULL	NULL	hookworm infection 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Field studies on different control schemes for hookworm infection ) .
	manualset3
265407	1	424307	15	NULL	NULL	NULL	NULL	consultants	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Better to increase number of consultants in accident and emergency medicine .
	manualset3
265408	2	424307	15	NULL	NULL	NULL	NULL	accident	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Better to increase number of consultants in accident and emergency medicine .
	manualset3
265409	3	424307	15	NULL	NULL	NULL	NULL	emergency medicine 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Better to increase number of consultants in accident and emergency medicine .
	manualset3
265410	1	424308	15	NULL	NULL	NULL	NULL	mental health	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Better mental health was significantly related to less fatigue ( Functional Assessment of Cancer Therapy ( FACT ) - fatigue , r = 0.61 , P & lt ; 0.0001 ) , less pain ( European Organisation for Research and Treatment of Cancer ( EORTC ) , r = -0.54 , P & lt ; 0.0001 ) , fewer stressful life events ( Life Event Scale , r = -0.44 , P ) 0.001 ) , and greater social support ( MOS Social Support Survey , r = 0.41 , P & lt ; 0.01 ) .
	manualset3
265411	2	424308	15	NULL	NULL	NULL	NULL	 fatigue	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Better mental health was significantly related to less fatigue ( Functional Assessment of Cancer Therapy ( FACT ) - fatigue , r = 0.61 , P & lt ; 0.0001 ) , less pain ( European Organisation for Research and Treatment of Cancer ( EORTC ) , r = -0.54 , P & lt ; 0.0001 ) , fewer stressful life events ( Life Event Scale , r = -0.44 , P ) 0.001 ) , and greater social support ( MOS Social Support Survey , r = 0.41 , P & lt ; 0.01 ) .
	manualset3
265412	3	424308	15	NULL	NULL	NULL	NULL	Functional Assessment of Cancer Therapy ( FACT ) 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Better mental health was significantly related to less fatigue ( Functional Assessment of Cancer Therapy ( FACT ) - fatigue , r = 0.61 , P & lt ; 0.0001 ) , less pain ( European Organisation for Research and Treatment of Cancer ( EORTC ) , r = -0.54 , P & lt ; 0.0001 ) , fewer stressful life events ( Life Event Scale , r = -0.44 , P ) 0.001 ) , and greater social support ( MOS Social Support Survey , r = 0.41 , P & lt ; 0.01 ) .
	manualset3
265413	4	424308	15	NULL	NULL	NULL	NULL	fatigue	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Better mental health was significantly related to less fatigue ( Functional Assessment of Cancer Therapy ( FACT ) - fatigue , r = 0.61 , P & lt ; 0.0001 ) , less pain ( European Organisation for Research and Treatment of Cancer ( EORTC ) , r = -0.54 , P & lt ; 0.0001 ) , fewer stressful life events ( Life Event Scale , r = -0.44 , P ) 0.001 ) , and greater social support ( MOS Social Support Survey , r = 0.41 , P & lt ; 0.01 ) .
	manualset3
265414	5	424308	15	NULL	NULL	NULL	NULL	r = 0.61	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Better mental health was significantly related to less fatigue ( Functional Assessment of Cancer Therapy ( FACT ) - fatigue , r = 0.61 , P & lt ; 0.0001 ) , less pain ( European Organisation for Research and Treatment of Cancer ( EORTC ) , r = -0.54 , P & lt ; 0.0001 ) , fewer stressful life events ( Life Event Scale , r = -0.44 , P ) 0.001 ) , and greater social support ( MOS Social Support Survey , r = 0.41 , P & lt ; 0.01 ) .
	manualset3
265415	6	424308	15	NULL	NULL	NULL	NULL	P & lt ; 0.0001	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Better mental health was significantly related to less fatigue ( Functional Assessment of Cancer Therapy ( FACT ) - fatigue , r = 0.61 , P & lt ; 0.0001 ) , less pain ( European Organisation for Research and Treatment of Cancer ( EORTC ) , r = -0.54 , P & lt ; 0.0001 ) , fewer stressful life events ( Life Event Scale , r = -0.44 , P ) 0.001 ) , and greater social support ( MOS Social Support Survey , r = 0.41 , P & lt ; 0.01 ) .
	manualset3
265416	7	424308	15	NULL	NULL	NULL	NULL	 pain	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Better mental health was significantly related to less fatigue ( Functional Assessment of Cancer Therapy ( FACT ) - fatigue , r = 0.61 , P & lt ; 0.0001 ) , less pain ( European Organisation for Research and Treatment of Cancer ( EORTC ) , r = -0.54 , P & lt ; 0.0001 ) , fewer stressful life events ( Life Event Scale , r = -0.44 , P ) 0.001 ) , and greater social support ( MOS Social Support Survey , r = 0.41 , P & lt ; 0.01 ) .
	manualset3
265417	8	424308	15	NULL	NULL	NULL	NULL	European Organisation for Research and Treatment of Cancer ( EORTC ) 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Better mental health was significantly related to less fatigue ( Functional Assessment of Cancer Therapy ( FACT ) - fatigue , r = 0.61 , P & lt ; 0.0001 ) , less pain ( European Organisation for Research and Treatment of Cancer ( EORTC ) , r = -0.54 , P & lt ; 0.0001 ) , fewer stressful life events ( Life Event Scale , r = -0.44 , P ) 0.001 ) , and greater social support ( MOS Social Support Survey , r = 0.41 , P & lt ; 0.01 ) .
	manualset3
265418	9	424308	15	NULL	NULL	NULL	NULL	r = -0.54	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Better mental health was significantly related to less fatigue ( Functional Assessment of Cancer Therapy ( FACT ) - fatigue , r = 0.61 , P & lt ; 0.0001 ) , less pain ( European Organisation for Research and Treatment of Cancer ( EORTC ) , r = -0.54 , P & lt ; 0.0001 ) , fewer stressful life events ( Life Event Scale , r = -0.44 , P ) 0.001 ) , and greater social support ( MOS Social Support Survey , r = 0.41 , P & lt ; 0.01 ) .
	manualset3
265419	10	424308	15	NULL	NULL	NULL	NULL	P & lt ; 0.0001	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Better mental health was significantly related to less fatigue ( Functional Assessment of Cancer Therapy ( FACT ) - fatigue , r = 0.61 , P & lt ; 0.0001 ) , less pain ( European Organisation for Research and Treatment of Cancer ( EORTC ) , r = -0.54 , P & lt ; 0.0001 ) , fewer stressful life events ( Life Event Scale , r = -0.44 , P ) 0.001 ) , and greater social support ( MOS Social Support Survey , r = 0.41 , P & lt ; 0.01 ) .
	manualset3
265420	11	424308	15	NULL	NULL	NULL	NULL	stressful life events	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Better mental health was significantly related to less fatigue ( Functional Assessment of Cancer Therapy ( FACT ) - fatigue , r = 0.61 , P & lt ; 0.0001 ) , less pain ( European Organisation for Research and Treatment of Cancer ( EORTC ) , r = -0.54 , P & lt ; 0.0001 ) , fewer stressful life events ( Life Event Scale , r = -0.44 , P ) 0.001 ) , and greater social support ( MOS Social Support Survey , r = 0.41 , P & lt ; 0.01 ) .
	manualset3
265421	12	424308	15	NULL	NULL	NULL	NULL	Life Event Scale	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Better mental health was significantly related to less fatigue ( Functional Assessment of Cancer Therapy ( FACT ) - fatigue , r = 0.61 , P & lt ; 0.0001 ) , less pain ( European Organisation for Research and Treatment of Cancer ( EORTC ) , r = -0.54 , P & lt ; 0.0001 ) , fewer stressful life events ( Life Event Scale , r = -0.44 , P ) 0.001 ) , and greater social support ( MOS Social Support Survey , r = 0.41 , P & lt ; 0.01 ) .
	manualset3
265422	13	424308	15	NULL	NULL	NULL	NULL	r = -0.44	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Better mental health was significantly related to less fatigue ( Functional Assessment of Cancer Therapy ( FACT ) - fatigue , r = 0.61 , P & lt ; 0.0001 ) , less pain ( European Organisation for Research and Treatment of Cancer ( EORTC ) , r = -0.54 , P & lt ; 0.0001 ) , fewer stressful life events ( Life Event Scale , r = -0.44 , P ) 0.001 ) , and greater social support ( MOS Social Support Survey , r = 0.41 , P & lt ; 0.01 ) .
	manualset3
265423	14	424308	15	NULL	NULL	NULL	NULL	P ) 0.001 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Better mental health was significantly related to less fatigue ( Functional Assessment of Cancer Therapy ( FACT ) - fatigue , r = 0.61 , P & lt ; 0.0001 ) , less pain ( European Organisation for Research and Treatment of Cancer ( EORTC ) , r = -0.54 , P & lt ; 0.0001 ) , fewer stressful life events ( Life Event Scale , r = -0.44 , P ) 0.001 ) , and greater social support ( MOS Social Support Survey , r = 0.41 , P & lt ; 0.01 ) .
	manualset3
265424	15	424308	15	NULL	NULL	NULL	NULL	social support	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Better mental health was significantly related to less fatigue ( Functional Assessment of Cancer Therapy ( FACT ) - fatigue , r = 0.61 , P & lt ; 0.0001 ) , less pain ( European Organisation for Research and Treatment of Cancer ( EORTC ) , r = -0.54 , P & lt ; 0.0001 ) , fewer stressful life events ( Life Event Scale , r = -0.44 , P ) 0.001 ) , and greater social support ( MOS Social Support Survey , r = 0.41 , P & lt ; 0.01 ) .
	manualset3
265425	16	424308	15	NULL	NULL	NULL	NULL	MOS Social Support Survey 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Better mental health was significantly related to less fatigue ( Functional Assessment of Cancer Therapy ( FACT ) - fatigue , r = 0.61 , P & lt ; 0.0001 ) , less pain ( European Organisation for Research and Treatment of Cancer ( EORTC ) , r = -0.54 , P & lt ; 0.0001 ) , fewer stressful life events ( Life Event Scale , r = -0.44 , P ) 0.001 ) , and greater social support ( MOS Social Support Survey , r = 0.41 , P & lt ; 0.01 ) .
	manualset3
265426	17	424308	15	NULL	NULL	NULL	NULL	r = 0.41	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Better mental health was significantly related to less fatigue ( Functional Assessment of Cancer Therapy ( FACT ) - fatigue , r = 0.61 , P & lt ; 0.0001 ) , less pain ( European Organisation for Research and Treatment of Cancer ( EORTC ) , r = -0.54 , P & lt ; 0.0001 ) , fewer stressful life events ( Life Event Scale , r = -0.44 , P ) 0.001 ) , and greater social support ( MOS Social Support Survey , r = 0.41 , P & lt ; 0.01 ) .
	manualset3
265427	18	424308	15	NULL	NULL	NULL	NULL	P & lt ; 0.01	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Better mental health was significantly related to less fatigue ( Functional Assessment of Cancer Therapy ( FACT ) - fatigue , r = 0.61 , P & lt ; 0.0001 ) , less pain ( European Organisation for Research and Treatment of Cancer ( EORTC ) , r = -0.54 , P & lt ; 0.0001 ) , fewer stressful life events ( Life Event Scale , r = -0.44 , P ) 0.001 ) , and greater social support ( MOS Social Support Survey , r = 0.41 , P & lt ; 0.01 ) .
	manualset3
265428	1	424309	15	NULL	NULL	NULL	NULL	1667-1815	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 1667-1815 the country was rule alternately by the Netherlands and Great Britian .
	manualset3
265429	2	424309	15	NULL	NULL	NULL	NULL	country	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 1667-1815 the country was rule alternately by the Netherlands and Great Britian .
	manualset3
265430	3	424309	15	NULL	NULL	NULL	NULL	Netherlands	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 1667-1815 the country was rule alternately by the Netherlands and Great Britian .
	manualset3
265431	4	424309	15	NULL	NULL	NULL	NULL	Great Britian	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 1667-1815 the country was rule alternately by the Netherlands and Great Britian .
	manualset3
265432	1	424310	15	NULL	NULL	NULL	NULL	Between 1979 and 1985	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 1979 and 1985 , 25 women aged 28-40 years of age underwent microsurgical tubotubal anastomosis at the University of Copenhagen 's Hvidovre Hospital for reversal of sterilization .
	manualset3
265433	2	424310	15	NULL	NULL	NULL	NULL	25 women	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 1979 and 1985 , 25 women aged 28-40 years of age underwent microsurgical tubotubal anastomosis at the University of Copenhagen 's Hvidovre Hospital for reversal of sterilization .
	manualset3
265434	3	424310	15	NULL	NULL	NULL	NULL	28-40 years	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 1979 and 1985 , 25 women aged 28-40 years of age underwent microsurgical tubotubal anastomosis at the University of Copenhagen 's Hvidovre Hospital for reversal of sterilization .
	manualset3
265435	4	424310	15	NULL	NULL	NULL	NULL	age 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 1979 and 1985 , 25 women aged 28-40 years of age underwent microsurgical tubotubal anastomosis at the University of Copenhagen 's Hvidovre Hospital for reversal of sterilization .
	manualset3
265436	5	424310	15	NULL	NULL	NULL	NULL	microsurgical tubotubal anastomosis	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 1979 and 1985 , 25 women aged 28-40 years of age underwent microsurgical tubotubal anastomosis at the University of Copenhagen 's Hvidovre Hospital for reversal of sterilization .
	manualset3
265437	6	424310	15	NULL	NULL	NULL	NULL	University of Copenhagen 's Hvidovre Hospital	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 1979 and 1985 , 25 women aged 28-40 years of age underwent microsurgical tubotubal anastomosis at the University of Copenhagen 's Hvidovre Hospital for reversal of sterilization .
	manualset3
265438	7	424310	15	NULL	NULL	NULL	NULL	reversal of sterilization	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 1979 and 1985 , 25 women aged 28-40 years of age underwent microsurgical tubotubal anastomosis at the University of Copenhagen 's Hvidovre Hospital for reversal of sterilization .
	manualset3
265439	1	424311	15	NULL	NULL	NULL	NULL	Between 1985 and 1990	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 1985 and 1990 , 43 men died of coronary heart disease .
	manualset3
265440	2	424311	15	NULL	NULL	NULL	NULL	43 men	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 1985 and 1990 , 43 men died of coronary heart disease .
	manualset3
265441	3	424311	15	NULL	NULL	NULL	NULL	coronary heart disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 1985 and 1990 , 43 men died of coronary heart disease .
	manualset3
265442	1	424312	15	NULL	NULL	NULL	NULL	Between 2004 and 2007	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 2004 and 2007 , Girls Incorporated conducted research about the experience of five affiliates from different parts of the United States as they engaged with girls in Girls Study Girls Inc. , a participatory evaluation project that explored the meaning and impact of Girls Inc. environments and uncovered ways such environments can be improved .
	manualset3
265443	2	424312	15	NULL	NULL	NULL	NULL	Girls	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 2004 and 2007 , Girls Incorporated conducted research about the experience of five affiliates from different parts of the United States as they engaged with girls in Girls Study Girls Inc. , a participatory evaluation project that explored the meaning and impact of Girls Inc. environments and uncovered ways such environments can be improved .
	manualset3
265444	3	424312	15	NULL	NULL	NULL	NULL	research	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 2004 and 2007 , Girls Incorporated conducted research about the experience of five affiliates from different parts of the United States as they engaged with girls in Girls Study Girls Inc. , a participatory evaluation project that explored the meaning and impact of Girls Inc. environments and uncovered ways such environments can be improved .
	manualset3
265445	4	424312	15	NULL	NULL	NULL	NULL	experience	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 2004 and 2007 , Girls Incorporated conducted research about the experience of five affiliates from different parts of the United States as they engaged with girls in Girls Study Girls Inc. , a participatory evaluation project that explored the meaning and impact of Girls Inc. environments and uncovered ways such environments can be improved .
	manualset3
265446	5	424312	15	NULL	NULL	NULL	NULL	five affiliates	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 2004 and 2007 , Girls Incorporated conducted research about the experience of five affiliates from different parts of the United States as they engaged with girls in Girls Study Girls Inc. , a participatory evaluation project that explored the meaning and impact of Girls Inc. environments and uncovered ways such environments can be improved .
	manualset3
265447	6	424312	15	NULL	NULL	NULL	NULL	different parts of the United States	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 2004 and 2007 , Girls Incorporated conducted research about the experience of five affiliates from different parts of the United States as they engaged with girls in Girls Study Girls Inc. , a participatory evaluation project that explored the meaning and impact of Girls Inc. environments and uncovered ways such environments can be improved .
	manualset3
265448	7	424312	15	NULL	NULL	NULL	NULL	girls	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 2004 and 2007 , Girls Incorporated conducted research about the experience of five affiliates from different parts of the United States as they engaged with girls in Girls Study Girls Inc. , a participatory evaluation project that explored the meaning and impact of Girls Inc. environments and uncovered ways such environments can be improved .
	manualset3
265449	8	424312	15	NULL	NULL	NULL	NULL	Girls Study Girls Inc	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 2004 and 2007 , Girls Incorporated conducted research about the experience of five affiliates from different parts of the United States as they engaged with girls in Girls Study Girls Inc. , a participatory evaluation project that explored the meaning and impact of Girls Inc. environments and uncovered ways such environments can be improved .
	manualset3
265450	9	424312	15	NULL	NULL	NULL	NULL	participatory evaluation project	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 2004 and 2007 , Girls Incorporated conducted research about the experience of five affiliates from different parts of the United States as they engaged with girls in Girls Study Girls Inc. , a participatory evaluation project that explored the meaning and impact of Girls Inc. environments and uncovered ways such environments can be improved .
	manualset3
265451	10	424312	15	NULL	NULL	NULL	NULL	meaning	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 2004 and 2007 , Girls Incorporated conducted research about the experience of five affiliates from different parts of the United States as they engaged with girls in Girls Study Girls Inc. , a participatory evaluation project that explored the meaning and impact of Girls Inc. environments and uncovered ways such environments can be improved .
	manualset3
265452	11	424312	15	NULL	NULL	NULL	NULL	impact of Girls Inc. environments 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 2004 and 2007 , Girls Incorporated conducted research about the experience of five affiliates from different parts of the United States as they engaged with girls in Girls Study Girls Inc. , a participatory evaluation project that explored the meaning and impact of Girls Inc. environments and uncovered ways such environments can be improved .
	manualset3
265453	12	424312	15	NULL	NULL	NULL	NULL	ways	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 2004 and 2007 , Girls Incorporated conducted research about the experience of five affiliates from different parts of the United States as they engaged with girls in Girls Study Girls Inc. , a participatory evaluation project that explored the meaning and impact of Girls Inc. environments and uncovered ways such environments can be improved .
	manualset3
265454	13	424312	15	NULL	NULL	NULL	NULL	environments	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 2004 and 2007 , Girls Incorporated conducted research about the experience of five affiliates from different parts of the United States as they engaged with girls in Girls Study Girls Inc. , a participatory evaluation project that explored the meaning and impact of Girls Inc. environments and uncovered ways such environments can be improved .
	manualset3
265455	1	424313	15	NULL	NULL	NULL	NULL	5mM glucose	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 5 and 20 mM glucose , the oxidative production of CO2 from ( 3 , 4-14C ) glucose represented close to 100 % of the total glucose utilization by the cells .
	manualset3
265456	2	424313	15	NULL	NULL	NULL	NULL	20 mM glucose	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 5 and 20 mM glucose , the oxidative production of CO2 from ( 3 , 4-14C ) glucose represented close to 100 % of the total glucose utilization by the cells .
	manualset3
265457	3	424313	15	NULL	NULL	NULL	NULL	oxidative production of CO2	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 5 and 20 mM glucose , the oxidative production of CO2 from ( 3 , 4-14C ) glucose represented close to 100 % of the total glucose utilization by the cells .
	manualset3
265458	4	424313	15	NULL	NULL	NULL	NULL	( 3 , 4-14C ) glucose	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 5 and 20 mM glucose , the oxidative production of CO2 from ( 3 , 4-14C ) glucose represented close to 100 % of the total glucose utilization by the cells .
	manualset3
265459	5	424313	15	NULL	NULL	NULL	NULL	100 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 5 and 20 mM glucose , the oxidative production of CO2 from ( 3 , 4-14C ) glucose represented close to 100 % of the total glucose utilization by the cells .
	manualset3
265460	6	424313	15	NULL	NULL	NULL	NULL	total glucose utilization	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 5 and 20 mM glucose , the oxidative production of CO2 from ( 3 , 4-14C ) glucose represented close to 100 % of the total glucose utilization by the cells .
	manualset3
265461	7	424313	15	NULL	NULL	NULL	NULL	cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 5 and 20 mM glucose , the oxidative production of CO2 from ( 3 , 4-14C ) glucose represented close to 100 % of the total glucose utilization by the cells .
	manualset3
265462	1	424314	15	NULL	NULL	NULL	NULL	7 kHz 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 7 and 8 kHz , both ZSC magnitude and angle decreased sharply with frequency , and both increased somewhat at higher frequencies .
	manualset3
265463	2	424314	15	NULL	NULL	NULL	NULL	8 kHz 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 7 and 8 kHz , both ZSC magnitude and angle decreased sharply with frequency , and both increased somewhat at higher frequencies .
	manualset3
265464	3	424314	15	NULL	NULL	NULL	NULL	ZSC magnitude	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 7 and 8 kHz , both ZSC magnitude and angle decreased sharply with frequency , and both increased somewhat at higher frequencies .
	manualset3
265465	4	424314	15	NULL	NULL	NULL	NULL	angle	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 7 and 8 kHz , both ZSC magnitude and angle decreased sharply with frequency , and both increased somewhat at higher frequencies .
	manualset3
265466	5	424314	15	NULL	NULL	NULL	NULL	frequency	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 7 and 8 kHz , both ZSC magnitude and angle decreased sharply with frequency , and both increased somewhat at higher frequencies .
	manualset3
265467	6	424314	15	NULL	NULL	NULL	NULL	frequencies	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between 7 and 8 kHz , both ZSC magnitude and angle decreased sharply with frequency , and both increased somewhat at higher frequencies .
	manualset3
265468	1	424315	15	NULL	NULL	NULL	NULL	Between February and April 1991	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between February and April 1991 , unusual numbers of bovine abortion around Antananarivo ( central highlands , Madagascar ) were reported by official veterinary services .
	manualset3
265469	2	424315	15	NULL	NULL	NULL	NULL	numbers	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between February and April 1991 , unusual numbers of bovine abortion around Antananarivo ( central highlands , Madagascar ) were reported by official veterinary services .
	manualset3
265470	3	424315	15	NULL	NULL	NULL	NULL	bovine abortion 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between February and April 1991 , unusual numbers of bovine abortion around Antananarivo ( central highlands , Madagascar ) were reported by official veterinary services .
	manualset3
265471	4	424315	15	NULL	NULL	NULL	NULL	Antananarivo	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between February and April 1991 , unusual numbers of bovine abortion around Antananarivo ( central highlands , Madagascar ) were reported by official veterinary services .
	manualset3
265472	5	424315	15	NULL	NULL	NULL	NULL	central highlands , Madagascar 	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between February and April 1991 , unusual numbers of bovine abortion around Antananarivo ( central highlands , Madagascar ) were reported by official veterinary services .
	manualset3
265473	6	424315	15	NULL	NULL	NULL	NULL	official veterinary services 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between February and April 1991 , unusual numbers of bovine abortion around Antananarivo ( central highlands , Madagascar ) were reported by official veterinary services .
	manualset3
265474	1	424316	15	NULL	NULL	NULL	NULL	Between September and December , 1996	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between September and December , 1996 , microbial contamination and water activity of in-use lubricants in sheathed and lubricated non-touch catheters connected to a tube used by 46 outpatients at our hospital was examined .
	manualset3
265475	2	424316	15	NULL	NULL	NULL	NULL	microbial contamination 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between September and December , 1996 , microbial contamination and water activity of in-use lubricants in sheathed and lubricated non-touch catheters connected to a tube used by 46 outpatients at our hospital was examined .
	manualset3
265476	3	424316	15	NULL	NULL	NULL	NULL	water activity 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between September and December , 1996 , microbial contamination and water activity of in-use lubricants in sheathed and lubricated non-touch catheters connected to a tube used by 46 outpatients at our hospital was examined .
	manualset3
265477	4	424316	15	NULL	NULL	NULL	NULL	in-use lubricants	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between September and December , 1996 , microbial contamination and water activity of in-use lubricants in sheathed and lubricated non-touch catheters connected to a tube used by 46 outpatients at our hospital was examined .
	manualset3
265478	5	424316	15	NULL	NULL	NULL	NULL	non-touch catheters 	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between September and December , 1996 , microbial contamination and water activity of in-use lubricants in sheathed and lubricated non-touch catheters connected to a tube used by 46 outpatients at our hospital was examined .
	manualset3
265479	6	424316	15	NULL	NULL	NULL	NULL	tube 	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between September and December , 1996 , microbial contamination and water activity of in-use lubricants in sheathed and lubricated non-touch catheters connected to a tube used by 46 outpatients at our hospital was examined .
	manualset3
265480	7	424316	15	NULL	NULL	NULL	NULL	46 outpatients 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between September and December , 1996 , microbial contamination and water activity of in-use lubricants in sheathed and lubricated non-touch catheters connected to a tube used by 46 outpatients at our hospital was examined .
	manualset3
265481	8	424316	15	NULL	NULL	NULL	NULL	hospital	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between September and December , 1996 , microbial contamination and water activity of in-use lubricants in sheathed and lubricated non-touch catheters connected to a tube used by 46 outpatients at our hospital was examined .
	manualset3
265495	1	424317	15	NULL	NULL	NULL	NULL	pH 3	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between pH 3 and 5 , glutamate adsorbs strongly , up to 1.4 micromol m ( -2 ) , and the adsorption decreases with increasing ionic strength .
	manualset3
265496	2	424317	15	NULL	NULL	NULL	NULL	pH 5 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between pH 3 and 5 , glutamate adsorbs strongly , up to 1.4 micromol m ( -2 ) , and the adsorption decreases with increasing ionic strength .
	manualset3
265497	3	424317	15	NULL	NULL	NULL	NULL	glutamate 	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between pH 3 and 5 , glutamate adsorbs strongly , up to 1.4 micromol m ( -2 ) , and the adsorption decreases with increasing ionic strength .
	manualset3
265498	4	424317	15	NULL	NULL	NULL	NULL	1.4 micromol m ( -2 ) 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between pH 3 and 5 , glutamate adsorbs strongly , up to 1.4 micromol m ( -2 ) , and the adsorption decreases with increasing ionic strength .
	manualset3
265499	5	424317	15	NULL	NULL	NULL	NULL	adsorption 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between pH 3 and 5 , glutamate adsorbs strongly , up to 1.4 micromol m ( -2 ) , and the adsorption decreases with increasing ionic strength .
	manualset3
265500	6	424317	15	NULL	NULL	NULL	NULL	ionic strength	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between pH 3 and 5 , glutamate adsorbs strongly , up to 1.4 micromol m ( -2 ) , and the adsorption decreases with increasing ionic strength .
	manualset3
265501	1	424318	15	NULL	NULL	NULL	NULL	Between the 51st and 119th days	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between the 51st and 119th days of their pregnancies , 5 of the 6 Hammondia-vaccinated does and the 2 controls were each inoculated orally with 1 , 000 infective oocysts of the GT-1 strain of T gondii .
	manualset3
265502	2	424318	15	NULL	NULL	NULL	NULL	pregnancies 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between the 51st and 119th days of their pregnancies , 5 of the 6 Hammondia-vaccinated does and the 2 controls were each inoculated orally with 1 , 000 infective oocysts of the GT-1 strain of T gondii .
	manualset3
265503	3	424318	15	NULL	NULL	NULL	NULL	5	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between the 51st and 119th days of their pregnancies , 5 of the 6 Hammondia-vaccinated does and the 2 controls were each inoculated orally with 1 , 000 infective oocysts of the GT-1 strain of T gondii .
	manualset3
265504	4	424318	15	NULL	NULL	NULL	NULL	6 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between the 51st and 119th days of their pregnancies , 5 of the 6 Hammondia-vaccinated does and the 2 controls were each inoculated orally with 1 , 000 infective oocysts of the GT-1 strain of T gondii .
	manualset3
265505	5	424318	15	NULL	NULL	NULL	NULL	Hammondia-vaccinated does	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between the 51st and 119th days of their pregnancies , 5 of the 6 Hammondia-vaccinated does and the 2 controls were each inoculated orally with 1 , 000 infective oocysts of the GT-1 strain of T gondii .
	manualset3
265506	6	424318	15	NULL	NULL	NULL	NULL	2 controls	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between the 51st and 119th days of their pregnancies , 5 of the 6 Hammondia-vaccinated does and the 2 controls were each inoculated orally with 1 , 000 infective oocysts of the GT-1 strain of T gondii .
	manualset3
265508	7	424318	15	NULL	NULL	NULL	NULL	1 , 000 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between the 51st and 119th days of their pregnancies , 5 of the 6 Hammondia-vaccinated does and the 2 controls were each inoculated orally with 1 , 000 infective oocysts of the GT-1 strain of T gondii .
	manualset3
265511	8	424318	15	NULL	NULL	NULL	NULL	infective oocysts	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between the 51st and 119th days of their pregnancies , 5 of the 6 Hammondia-vaccinated does and the 2 controls were each inoculated orally with 1 , 000 infective oocysts of the GT-1 strain of T gondii .
	manualset3
265513	9	424318	15	NULL	NULL	NULL	NULL	GT-1 strain of T gondii	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Between the 51st and 119th days of their pregnancies , 5 of the 6 Hammondia-vaccinated does and the 2 controls were each inoculated orally with 1 , 000 infective oocysts of the GT-1 strain of T gondii .
	manualset3
265514	1	424319	15	NULL	NULL	NULL	NULL	traditional training	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Beyond the traditional training , the authors underline the importance of self-training inscribed in the daily life of every health worker with a genuine help-relationship .
	manualset3
265515	2	424319	15	NULL	NULL	NULL	NULL	authors	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Beyond the traditional training , the authors underline the importance of self-training inscribed in the daily life of every health worker with a genuine help-relationship .
	manualset3
265527	3	424319	15	NULL	NULL	NULL	NULL	importance 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Beyond the traditional training , the authors underline the importance of self-training inscribed in the daily life of every health worker with a genuine help-relationship .
	manualset3
265529	4	424319	15	NULL	NULL	NULL	NULL	self-training	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Beyond the traditional training , the authors underline the importance of self-training inscribed in the daily life of every health worker with a genuine help-relationship .
	manualset3
265531	5	424319	15	NULL	NULL	NULL	NULL	daily life	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Beyond the traditional training , the authors underline the importance of self-training inscribed in the daily life of every health worker with a genuine help-relationship .
	manualset3
265532	6	424319	15	NULL	NULL	NULL	NULL	health worker	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Beyond the traditional training , the authors underline the importance of self-training inscribed in the daily life of every health worker with a genuine help-relationship .
	manualset3
265534	7	424319	15	NULL	NULL	NULL	NULL	genuine help-relationship	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Beyond the traditional training , the authors underline the importance of self-training inscribed in the daily life of every health worker with a genuine help-relationship .
	manualset3
265537	1	424320	15	NULL	NULL	NULL	NULL	Bicarbonate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bicarbonate was shown to effect the transport of sulfate , where uptake was accelerated by intracellular bicarbonate and competitively inhibited by extracellular bicarbonate .
	manualset3
265539	2	424320	15	NULL	NULL	NULL	NULL	transport of sulfate	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bicarbonate was shown to effect the transport of sulfate , where uptake was accelerated by intracellular bicarbonate and competitively inhibited by extracellular bicarbonate .
	manualset3
265542	3	424320	15	NULL	NULL	NULL	NULL	uptake	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bicarbonate was shown to effect the transport of sulfate , where uptake was accelerated by intracellular bicarbonate and competitively inhibited by extracellular bicarbonate .
	manualset3
265544	4	424320	15	NULL	NULL	NULL	NULL	intracellular bicarbonate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bicarbonate was shown to effect the transport of sulfate , where uptake was accelerated by intracellular bicarbonate and competitively inhibited by extracellular bicarbonate .
	manualset3
265547	5	424320	15	NULL	NULL	NULL	NULL	extracellular bicarbonate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bicarbonate was shown to effect the transport of sulfate , where uptake was accelerated by intracellular bicarbonate and competitively inhibited by extracellular bicarbonate .
	manualset3
265552	1	424321	15	NULL	NULL	NULL	NULL	Bidirectional transport studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bidirectional transport studies of 5 microM loperamide showed efflux to be fivefold higher than influx ( 42 x 10 ( -6 ) compared to 8 x 10 ( -6 ) cm/s ) ; however , this decreased to twofold at 10 microM and was abolished using 100 microM loperamide .
	manualset3
265554	2	424321	15	NULL	NULL	NULL	NULL	5 microM	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bidirectional transport studies of 5 microM loperamide showed efflux to be fivefold higher than influx ( 42 x 10 ( -6 ) compared to 8 x 10 ( -6 ) cm/s ) ; however , this decreased to twofold at 10 microM and was abolished using 100 microM loperamide .
	manualset3
265556	3	424321	15	NULL	NULL	NULL	NULL	loperamide	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bidirectional transport studies of 5 microM loperamide showed efflux to be fivefold higher than influx ( 42 x 10 ( -6 ) compared to 8 x 10 ( -6 ) cm/s ) ; however , this decreased to twofold at 10 microM and was abolished using 100 microM loperamide .
	manualset3
265559	4	424321	15	NULL	NULL	NULL	NULL	efflux	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bidirectional transport studies of 5 microM loperamide showed efflux to be fivefold higher than influx ( 42 x 10 ( -6 ) compared to 8 x 10 ( -6 ) cm/s ) ; however , this decreased to twofold at 10 microM and was abolished using 100 microM loperamide .
	manualset3
265561	5	424321	15	NULL	NULL	NULL	NULL	influx 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bidirectional transport studies of 5 microM loperamide showed efflux to be fivefold higher than influx ( 42 x 10 ( -6 ) compared to 8 x 10 ( -6 ) cm/s ) ; however , this decreased to twofold at 10 microM and was abolished using 100 microM loperamide .
	manualset3
265563	6	424321	15	NULL	NULL	NULL	NULL	42 x 10 ( -6 ) cm/s	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bidirectional transport studies of 5 microM loperamide showed efflux to be fivefold higher than influx ( 42 x 10 ( -6 ) compared to 8 x 10 ( -6 ) cm/s ) ; however , this decreased to twofold at 10 microM and was abolished using 100 microM loperamide .
	manualset3
265564	7	424321	15	NULL	NULL	NULL	NULL	8 x 10 ( -6 ) cm/s 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bidirectional transport studies of 5 microM loperamide showed efflux to be fivefold higher than influx ( 42 x 10 ( -6 ) compared to 8 x 10 ( -6 ) cm/s ) ; however , this decreased to twofold at 10 microM and was abolished using 100 microM loperamide .
	manualset3
265565	8	424321	15	NULL	NULL	NULL	NULL	10 microM	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bidirectional transport studies of 5 microM loperamide showed efflux to be fivefold higher than influx ( 42 x 10 ( -6 ) compared to 8 x 10 ( -6 ) cm/s ) ; however , this decreased to twofold at 10 microM and was abolished using 100 microM loperamide .
	manualset3
265566	9	424321	15	NULL	NULL	NULL	NULL	100 microM	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bidirectional transport studies of 5 microM loperamide showed efflux to be fivefold higher than influx ( 42 x 10 ( -6 ) compared to 8 x 10 ( -6 ) cm/s ) ; however , this decreased to twofold at 10 microM and was abolished using 100 microM loperamide .
	manualset3
265568	10	424321	15	NULL	NULL	NULL	NULL	loperamide	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bidirectional transport studies of 5 microM loperamide showed efflux to be fivefold higher than influx ( 42 x 10 ( -6 ) compared to 8 x 10 ( -6 ) cm/s ) ; however , this decreased to twofold at 10 microM and was abolished using 100 microM loperamide .
	manualset3
265570	1	424322	15	NULL	NULL	NULL	NULL	Bifid T waves	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bifid T waves occurred in 16 % of 600 normal children , 92 % of 37 cases of childhood ventricular septal defect ( VSD ) , 6 of 10 cases of tetralogy of Fallot ( children ) and 33 % of 193 patients with cerebrovascular accidents ( including 3 children ) .
	manualset3
265571	2	424322	15	NULL	NULL	NULL	NULL	16 % 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bifid T waves occurred in 16 % of 600 normal children , 92 % of 37 cases of childhood ventricular septal defect ( VSD ) , 6 of 10 cases of tetralogy of Fallot ( children ) and 33 % of 193 patients with cerebrovascular accidents ( including 3 children ) .
	manualset3
265572	3	424322	15	NULL	NULL	NULL	NULL	600 normal children	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bifid T waves occurred in 16 % of 600 normal children , 92 % of 37 cases of childhood ventricular septal defect ( VSD ) , 6 of 10 cases of tetralogy of Fallot ( children ) and 33 % of 193 patients with cerebrovascular accidents ( including 3 children ) .
	manualset3
265573	4	424322	15	NULL	NULL	NULL	NULL	92 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bifid T waves occurred in 16 % of 600 normal children , 92 % of 37 cases of childhood ventricular septal defect ( VSD ) , 6 of 10 cases of tetralogy of Fallot ( children ) and 33 % of 193 patients with cerebrovascular accidents ( including 3 children ) .
	manualset3
265574	5	424322	15	NULL	NULL	NULL	NULL	37 cases 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bifid T waves occurred in 16 % of 600 normal children , 92 % of 37 cases of childhood ventricular septal defect ( VSD ) , 6 of 10 cases of tetralogy of Fallot ( children ) and 33 % of 193 patients with cerebrovascular accidents ( including 3 children ) .
	manualset3
265575	6	424322	15	NULL	NULL	NULL	NULL	childhood ventricular septal defect ( VSD )	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bifid T waves occurred in 16 % of 600 normal children , 92 % of 37 cases of childhood ventricular septal defect ( VSD ) , 6 of 10 cases of tetralogy of Fallot ( children ) and 33 % of 193 patients with cerebrovascular accidents ( including 3 children ) .
	manualset3
265576	7	424322	15	NULL	NULL	NULL	NULL	6 of 10 cases	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bifid T waves occurred in 16 % of 600 normal children , 92 % of 37 cases of childhood ventricular septal defect ( VSD ) , 6 of 10 cases of tetralogy of Fallot ( children ) and 33 % of 193 patients with cerebrovascular accidents ( including 3 children ) .
	manualset3
265577	8	424322	15	NULL	NULL	NULL	NULL	tetralogy of Fallot ( children )	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bifid T waves occurred in 16 % of 600 normal children , 92 % of 37 cases of childhood ventricular septal defect ( VSD ) , 6 of 10 cases of tetralogy of Fallot ( children ) and 33 % of 193 patients with cerebrovascular accidents ( including 3 children ) .
	manualset3
265578	9	424322	15	NULL	NULL	NULL	NULL	 33 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bifid T waves occurred in 16 % of 600 normal children , 92 % of 37 cases of childhood ventricular septal defect ( VSD ) , 6 of 10 cases of tetralogy of Fallot ( children ) and 33 % of 193 patients with cerebrovascular accidents ( including 3 children ) .
	manualset3
265579	10	424322	15	NULL	NULL	NULL	NULL	193 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bifid T waves occurred in 16 % of 600 normal children , 92 % of 37 cases of childhood ventricular septal defect ( VSD ) , 6 of 10 cases of tetralogy of Fallot ( children ) and 33 % of 193 patients with cerebrovascular accidents ( including 3 children ) .
	manualset3
265580	11	424322	15	NULL	NULL	NULL	NULL	cerebrovascular accidents	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bifid T waves occurred in 16 % of 600 normal children , 92 % of 37 cases of childhood ventricular septal defect ( VSD ) , 6 of 10 cases of tetralogy of Fallot ( children ) and 33 % of 193 patients with cerebrovascular accidents ( including 3 children ) .
	manualset3
265581	12	424322	15	NULL	NULL	NULL	NULL	 3 children	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bifid T waves occurred in 16 % of 600 normal children , 92 % of 37 cases of childhood ventricular septal defect ( VSD ) , 6 of 10 cases of tetralogy of Fallot ( children ) and 33 % of 193 patients with cerebrovascular accidents ( including 3 children ) .
	manualset3
265582	1	424323	15	NULL	NULL	NULL	NULL	Firework injuries 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Firework injuries in Denmark in the period 1995/1996 to 2006/2007 ) .
	manualset3
265583	2	424323	15	NULL	NULL	NULL	NULL	Denmark 	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Firework injuries in Denmark in the period 1995/1996 to 2006/2007 ) .
	manualset3
265584	3	424323	15	NULL	NULL	NULL	NULL	period	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Firework injuries in Denmark in the period 1995/1996 to 2006/2007 ) .
	manualset3
265585	4	424323	15	NULL	NULL	NULL	NULL	1995/1996 to 2006/2007 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Firework injuries in Denmark in the period 1995/1996 to 2006/2007 ) .
	manualset3
265586	1	424324	15	NULL	NULL	NULL	NULL	Bilateral degenerative joint disease 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bilateral degenerative joint disease was noted in 8/16 ( 50 % ) .
	manualset3
265587	2	424324	15	NULL	NULL	NULL	NULL	8/16 ( 50 % )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bilateral degenerative joint disease was noted in 8/16 ( 50 % ) .
	manualset3
265588	1	424325	15	NULL	NULL	NULL	NULL	Bile duct-cannulated female Sprague-Dawley rats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bile duct-cannulated female and male Sprague-Dawley rats were gavaged with vehicle or with 25 or 50 mg ( 14C ) DAPM/kg , and bile was collected for 6 h. Serum and bile indicators of hepatobiliary toxicity were assessed , and radioactivity was measured in bile , serum , urine , and liver .
	manualset3
265589	2	424325	15	NULL	NULL	NULL	NULL	male Sprague-Dawley rats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bile duct-cannulated female and male Sprague-Dawley rats were gavaged with vehicle or with 25 or 50 mg ( 14C ) DAPM/kg , and bile was collected for 6 h. Serum and bile indicators of hepatobiliary toxicity were assessed , and radioactivity was measured in bile , serum , urine , and liver .
	manualset3
265590	3	424325	15	NULL	NULL	NULL	NULL	 vehicle	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bile duct-cannulated female and male Sprague-Dawley rats were gavaged with vehicle or with 25 or 50 mg ( 14C ) DAPM/kg , and bile was collected for 6 h. Serum and bile indicators of hepatobiliary toxicity were assessed , and radioactivity was measured in bile , serum , urine , and liver .
	manualset3
265591	4	424325	15	NULL	NULL	NULL	NULL	25 mg ( 14C ) DAPM/kg	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bile duct-cannulated female and male Sprague-Dawley rats were gavaged with vehicle or with 25 or 50 mg ( 14C ) DAPM/kg , and bile was collected for 6 h. Serum and bile indicators of hepatobiliary toxicity were assessed , and radioactivity was measured in bile , serum , urine , and liver .
	manualset3
265592	5	424325	15	NULL	NULL	NULL	NULL	50 mg ( 14C ) DAPM/kg 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bile duct-cannulated female and male Sprague-Dawley rats were gavaged with vehicle or with 25 or 50 mg ( 14C ) DAPM/kg , and bile was collected for 6 h. Serum and bile indicators of hepatobiliary toxicity were assessed , and radioactivity was measured in bile , serum , urine , and liver .
	manualset3
265593	6	424325	15	NULL	NULL	NULL	NULL	bile 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bile duct-cannulated female and male Sprague-Dawley rats were gavaged with vehicle or with 25 or 50 mg ( 14C ) DAPM/kg , and bile was collected for 6 h. Serum and bile indicators of hepatobiliary toxicity were assessed , and radioactivity was measured in bile , serum , urine , and liver .
	manualset3
265594	7	424325	15	NULL	NULL	NULL	NULL	6 h	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bile duct-cannulated female and male Sprague-Dawley rats were gavaged with vehicle or with 25 or 50 mg ( 14C ) DAPM/kg , and bile was collected for 6 h. Serum and bile indicators of hepatobiliary toxicity were assessed , and radioactivity was measured in bile , serum , urine , and liver .
	manualset3
265595	8	424325	15	NULL	NULL	NULL	NULL	Serum indicators	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bile duct-cannulated female and male Sprague-Dawley rats were gavaged with vehicle or with 25 or 50 mg ( 14C ) DAPM/kg , and bile was collected for 6 h. Serum and bile indicators of hepatobiliary toxicity were assessed , and radioactivity was measured in bile , serum , urine , and liver .
	manualset3
265596	9	424325	15	NULL	NULL	NULL	NULL	bile indicators	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bile duct-cannulated female and male Sprague-Dawley rats were gavaged with vehicle or with 25 or 50 mg ( 14C ) DAPM/kg , and bile was collected for 6 h. Serum and bile indicators of hepatobiliary toxicity were assessed , and radioactivity was measured in bile , serum , urine , and liver .
	manualset3
265597	10	424325	15	NULL	NULL	NULL	NULL	hepatobiliary toxicity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bile duct-cannulated female and male Sprague-Dawley rats were gavaged with vehicle or with 25 or 50 mg ( 14C ) DAPM/kg , and bile was collected for 6 h. Serum and bile indicators of hepatobiliary toxicity were assessed , and radioactivity was measured in bile , serum , urine , and liver .
	manualset3
265598	11	424325	15	NULL	NULL	NULL	NULL	radioactivity	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bile duct-cannulated female and male Sprague-Dawley rats were gavaged with vehicle or with 25 or 50 mg ( 14C ) DAPM/kg , and bile was collected for 6 h. Serum and bile indicators of hepatobiliary toxicity were assessed , and radioactivity was measured in bile , serum , urine , and liver .
	manualset3
265599	12	424325	15	NULL	NULL	NULL	NULL	bile	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bile duct-cannulated female and male Sprague-Dawley rats were gavaged with vehicle or with 25 or 50 mg ( 14C ) DAPM/kg , and bile was collected for 6 h. Serum and bile indicators of hepatobiliary toxicity were assessed , and radioactivity was measured in bile , serum , urine , and liver .
	manualset3
265600	13	424325	15	NULL	NULL	NULL	NULL	serum	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bile duct-cannulated female and male Sprague-Dawley rats were gavaged with vehicle or with 25 or 50 mg ( 14C ) DAPM/kg , and bile was collected for 6 h. Serum and bile indicators of hepatobiliary toxicity were assessed , and radioactivity was measured in bile , serum , urine , and liver .
	manualset3
265601	14	424325	15	NULL	NULL	NULL	NULL	urine	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bile duct-cannulated female and male Sprague-Dawley rats were gavaged with vehicle or with 25 or 50 mg ( 14C ) DAPM/kg , and bile was collected for 6 h. Serum and bile indicators of hepatobiliary toxicity were assessed , and radioactivity was measured in bile , serum , urine , and liver .
	manualset3
265602	15	424325	15	NULL	NULL	NULL	NULL	liver 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bile duct-cannulated female and male Sprague-Dawley rats were gavaged with vehicle or with 25 or 50 mg ( 14C ) DAPM/kg , and bile was collected for 6 h. Serum and bile indicators of hepatobiliary toxicity were assessed , and radioactivity was measured in bile , serum , urine , and liver .
	manualset3
265603	1	424326	15	NULL	NULL	NULL	NULL	Bile acids	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bile acids are cholesterol derivatives that are first synthesized in the liver ( primary bile acids ) and then metabolized by intestinal bacteria giving rise to secondary bile acids .
	manualset3
265604	2	424326	15	NULL	NULL	NULL	NULL	cholesterol derivatives	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bile acids are cholesterol derivatives that are first synthesized in the liver ( primary bile acids ) and then metabolized by intestinal bacteria giving rise to secondary bile acids .
	manualset3
265605	3	424326	15	NULL	NULL	NULL	NULL	liver	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bile acids are cholesterol derivatives that are first synthesized in the liver ( primary bile acids ) and then metabolized by intestinal bacteria giving rise to secondary bile acids .
	manualset3
265606	4	424326	15	NULL	NULL	NULL	NULL	primary bile acids 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bile acids are cholesterol derivatives that are first synthesized in the liver ( primary bile acids ) and then metabolized by intestinal bacteria giving rise to secondary bile acids .
	manualset3
265607	5	424326	15	NULL	NULL	NULL	NULL	intestinal bacteria	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bile acids are cholesterol derivatives that are first synthesized in the liver ( primary bile acids ) and then metabolized by intestinal bacteria giving rise to secondary bile acids .
	manualset3
265608	6	424326	15	NULL	NULL	NULL	NULL	secondary bile acids	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bile acids are cholesterol derivatives that are first synthesized in the liver ( primary bile acids ) and then metabolized by intestinal bacteria giving rise to secondary bile acids .
	manualset3
265659	1	424327	15	NULL	NULL	NULL	NULL	Bile salt 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bile salt , fat , water , and vitamin B 12 excretion after ileostomy .
	manualset3
265660	2	424327	15	NULL	NULL	NULL	NULL	fat	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bile salt , fat , water , and vitamin B 12 excretion after ileostomy .
	manualset3
265661	3	424327	15	NULL	NULL	NULL	NULL	water	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bile salt , fat , water , and vitamin B 12 excretion after ileostomy .
	manualset3
265662	4	424327	15	NULL	NULL	NULL	NULL	vitamin B 12 excretion 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bile salt , fat , water , and vitamin B 12 excretion after ileostomy .
	manualset3
265663	5	424327	15	NULL	NULL	NULL	NULL	ileostomy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Bile salt , fat , water , and vitamin B 12 excretion after ileostomy .
	manualset3
265664	1	424328	15	NULL	NULL	NULL	NULL	Biliary GSSG	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Biliary GSSG and GSH efflux rates were reduced and the GSSG-to-GSH ratio was not altered in controls and BCNU-treated rats at any time during ischemia and reperfusion .
	manualset3
265666	2	424328	15	NULL	NULL	NULL	NULL	GSH efflux rates 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Biliary GSSG and GSH efflux rates were reduced and the GSSG-to-GSH ratio was not altered in controls and BCNU-treated rats at any time during ischemia and reperfusion .
	manualset3
265668	3	424328	15	NULL	NULL	NULL	NULL	GSSG-to-GSH ratio	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Biliary GSSG and GSH efflux rates were reduced and the GSSG-to-GSH ratio was not altered in controls and BCNU-treated rats at any time during ischemia and reperfusion .
	manualset3
265669	4	424328	15	NULL	NULL	NULL	NULL	controls	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Biliary GSSG and GSH efflux rates were reduced and the GSSG-to-GSH ratio was not altered in controls and BCNU-treated rats at any time during ischemia and reperfusion .
	manualset3
265670	5	424328	15	NULL	NULL	NULL	NULL	BCNU-treated rats 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Biliary GSSG and GSH efflux rates were reduced and the GSSG-to-GSH ratio was not altered in controls and BCNU-treated rats at any time during ischemia and reperfusion .
	manualset3
265671	6	424328	15	NULL	NULL	NULL	NULL	time	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Biliary GSSG and GSH efflux rates were reduced and the GSSG-to-GSH ratio was not altered in controls and BCNU-treated rats at any time during ischemia and reperfusion .
	manualset3
265672	7	424328	15	NULL	NULL	NULL	NULL	ischemia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Biliary GSSG and GSH efflux rates were reduced and the GSSG-to-GSH ratio was not altered in controls and BCNU-treated rats at any time during ischemia and reperfusion .
	manualset3
265673	8	424328	15	NULL	NULL	NULL	NULL	reperfusion	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Biliary GSSG and GSH efflux rates were reduced and the GSSG-to-GSH ratio was not altered in controls and BCNU-treated rats at any time during ischemia and reperfusion .
	manualset3
265674	1	424329	15	NULL	NULL	NULL	NULL	Biliary MTX levels	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Biliary MTX levels in one patient undergoing intermediate dose MTX therapy ( 500 mg/m2 ) were measured by HPLC .
	manualset3
265675	2	424329	15	NULL	NULL	NULL	NULL	one 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Biliary MTX levels in one patient undergoing intermediate dose MTX therapy ( 500 mg/m2 ) were measured by HPLC .
	manualset3
265676	3	424329	15	NULL	NULL	NULL	NULL	patient 	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Biliary MTX levels in one patient undergoing intermediate dose MTX therapy ( 500 mg/m2 ) were measured by HPLC .
	manualset3
265677	4	424329	15	NULL	NULL	NULL	NULL	intermediate dose MTX therapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Biliary MTX levels in one patient undergoing intermediate dose MTX therapy ( 500 mg/m2 ) were measured by HPLC .
	manualset3
265678	5	424329	15	NULL	NULL	NULL	NULL	500 mg/m2	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Biliary MTX levels in one patient undergoing intermediate dose MTX therapy ( 500 mg/m2 ) were measured by HPLC .
	manualset3
265679	6	424329	15	NULL	NULL	NULL	NULL	HPLC	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Biliary MTX levels in one patient undergoing intermediate dose MTX therapy ( 500 mg/m2 ) were measured by HPLC .
	manualset3
265683	1	424330	15	NULL	NULL	NULL	NULL	First drafts	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( First drafts of the Environmental Health Criteria ( EHC ) circulated for comments by IPCS in 1994-1995 ) .
	manualset3
265684	2	424330	15	NULL	NULL	NULL	NULL	Environmental Health Criteria ( EHC )	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( First drafts of the Environmental Health Criteria ( EHC ) circulated for comments by IPCS in 1994-1995 ) .
	manualset3
265686	3	424330	15	NULL	NULL	NULL	NULL	comments	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( First drafts of the Environmental Health Criteria ( EHC ) circulated for comments by IPCS in 1994-1995 ) .
	manualset3
265693	4	424330	15	NULL	NULL	NULL	NULL	IPCS 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( First drafts of the Environmental Health Criteria ( EHC ) circulated for comments by IPCS in 1994-1995 ) .
	manualset3
265695	5	424330	15	NULL	NULL	NULL	NULL	1994-1995	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( First drafts of the Environmental Health Criteria ( EHC ) circulated for comments by IPCS in 1994-1995 ) .
	manualset3
245678	1	425331	7	NULL	NULL	0	NULL	Clusterin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Clusterin , also known as sulphated glycoprotein-2 or testosterone-repressed prostate message-2 , is a ubiquitous protein found in a variety of tissues and species .
	manualset3
245679	2	425331	7	NULL	NULL	0	NULL	sulphated glycoprotein-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Clusterin , also known as sulphated glycoprotein-2 or testosterone-repressed prostate message-2 , is a ubiquitous protein found in a variety of tissues and species .
	manualset3
245681	3	425331	7	NULL	NULL	0	NULL	testosterone-repressed prostate message-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Clusterin , also known as sulphated glycoprotein-2 or testosterone-repressed prostate message-2 , is a ubiquitous protein found in a variety of tissues and species .
	manualset3
245682	4	425331	7	NULL	NULL	0	NULL	 ubiquitous protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Clusterin , also known as sulphated glycoprotein-2 or testosterone-repressed prostate message-2 , is a ubiquitous protein found in a variety of tissues and species .
	manualset3
245684	5	425331	7	NULL	NULL	0	NULL	 tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Clusterin , also known as sulphated glycoprotein-2 or testosterone-repressed prostate message-2 , is a ubiquitous protein found in a variety of tissues and species .
	manualset3
245685	6	425331	7	NULL	NULL	0	NULL	species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Clusterin , also known as sulphated glycoprotein-2 or testosterone-repressed prostate message-2 , is a ubiquitous protein found in a variety of tissues and species .
	manualset3
245687	1	425332	7	NULL	NULL	0	NULL	Clusterin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Clusterin is a ubiquitous secretory sulfated glycoprotein .
	manualset3
245689	2	425332	7	NULL	NULL	0	NULL	secretory sulfated glycoprotein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Clusterin is a ubiquitous secretory sulfated glycoprotein .
	manualset3
245872	1	425333	7	NULL	NULL	0	NULL	Co-administration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-administration of the plant extract suppressed the elevation of lipid peroxidation , restored the reduced glutathion , and enhanced the superoxide dismutase activity .
	manualset3
245873	2	425333	7	NULL	NULL	0	NULL	plant extract 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-administration of the plant extract suppressed the elevation of lipid peroxidation , restored the reduced glutathion , and enhanced the superoxide dismutase activity .
	manualset3
245874	3	425333	7	NULL	NULL	0	NULL	elevation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-administration of the plant extract suppressed the elevation of lipid peroxidation , restored the reduced glutathion , and enhanced the superoxide dismutase activity .
	manualset3
245875	4	425333	7	NULL	NULL	0	NULL	lipid peroxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-administration of the plant extract suppressed the elevation of lipid peroxidation , restored the reduced glutathion , and enhanced the superoxide dismutase activity .
	manualset3
245876	5	425333	7	NULL	NULL	0	NULL	reduced glutathion	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-administration of the plant extract suppressed the elevation of lipid peroxidation , restored the reduced glutathion , and enhanced the superoxide dismutase activity .
	manualset3
245877	6	425333	7	NULL	NULL	0	NULL	superoxide dismutase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-administration of the plant extract suppressed the elevation of lipid peroxidation , restored the reduced glutathion , and enhanced the superoxide dismutase activity .
	manualset3
245878	1	425334	7	NULL	NULL	0	NULL	Co-circulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-circulation HIV-1 subtypes B , C , and CRF31_BC in a drug-nave population from Southernmost Brazil : analysis of primary resistance mutations .
	manualset3
245879	2	425334	7	NULL	NULL	0	NULL	HIV-1 subtypes B	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-circulation HIV-1 subtypes B , C , and CRF31_BC in a drug-nave population from Southernmost Brazil : analysis of primary resistance mutations .
	manualset3
245880	3	425334	7	NULL	NULL	0	NULL	HIV-1 subtypes C	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-circulation HIV-1 subtypes B , C , and CRF31_BC in a drug-nave population from Southernmost Brazil : analysis of primary resistance mutations .
	manualset3
245881	4	425334	7	NULL	NULL	0	NULL	CRF31_BC	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-circulation HIV-1 subtypes B , C , and CRF31_BC in a drug-nave population from Southernmost Brazil : analysis of primary resistance mutations .
	manualset3
245882	5	425334	7	NULL	NULL	0	NULL	drug-nave population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-circulation HIV-1 subtypes B , C , and CRF31_BC in a drug-nave population from Southernmost Brazil : analysis of primary resistance mutations .
	manualset3
245883	6	425334	7	NULL	NULL	0	NULL	Southernmost Brazil 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-circulation HIV-1 subtypes B , C , and CRF31_BC in a drug-nave population from Southernmost Brazil : analysis of primary resistance mutations .
	manualset3
245884	7	425334	7	NULL	NULL	0	NULL	analysis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-circulation HIV-1 subtypes B , C , and CRF31_BC in a drug-nave population from Southernmost Brazil : analysis of primary resistance mutations .
	manualset3
245885	8	425334	7	NULL	NULL	0	NULL	primary resistance mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-circulation HIV-1 subtypes B , C , and CRF31_BC in a drug-nave population from Southernmost Brazil : analysis of primary resistance mutations .
	manualset3
245886	1	425335	7	NULL	NULL	0	NULL	Co-evolution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-evolution of phases and connection strengths in a network of phase oscillators .
	manualset3
245887	2	425335	7	NULL	NULL	0	NULL	phases	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-evolution of phases and connection strengths in a network of phase oscillators .
	manualset3
245888	3	425335	7	NULL	NULL	0	NULL	connection strengths	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-evolution of phases and connection strengths in a network of phase oscillators .
	manualset3
245889	4	425335	7	NULL	NULL	0	NULL	network	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-evolution of phases and connection strengths in a network of phase oscillators .
	manualset3
245890	5	425335	7	NULL	NULL	NULL	NULL	 phase oscillators	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Co-evolution of phases and connection strengths in a network of phase oscillators .
	manualset3
245891	1	425336	7	NULL	NULL	0	NULL	Co-expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-expression of syntaxin 1A inhibits cAMP-stimulated current and capacitance changes in CFTR expressing cells and blocks cAMP-induced increases in cell surface CFTR .
	manualset3
245892	2	425336	7	NULL	NULL	0	NULL	syntaxin 1A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-expression of syntaxin 1A inhibits cAMP-stimulated current and capacitance changes in CFTR expressing cells and blocks cAMP-induced increases in cell surface CFTR .
	manualset3
245893	3	425336	7	NULL	NULL	0	NULL	cAMP-stimulated current changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-expression of syntaxin 1A inhibits cAMP-stimulated current and capacitance changes in CFTR expressing cells and blocks cAMP-induced increases in cell surface CFTR .
	manualset3
245894	4	425336	7	NULL	NULL	0	NULL	capacitance changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-expression of syntaxin 1A inhibits cAMP-stimulated current and capacitance changes in CFTR expressing cells and blocks cAMP-induced increases in cell surface CFTR .
	manualset3
245895	5	425336	7	NULL	NULL	0	NULL	CFTR expressing cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-expression of syntaxin 1A inhibits cAMP-stimulated current and capacitance changes in CFTR expressing cells and blocks cAMP-induced increases in cell surface CFTR .
	manualset3
245896	6	425336	7	NULL	NULL	0	NULL	cell surface CFTR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-expression of syntaxin 1A inhibits cAMP-stimulated current and capacitance changes in CFTR expressing cells and blocks cAMP-induced increases in cell surface CFTR .
	manualset3
249463	7	425336	7	NULL	NULL	0	NULL	 cAMP-induced increases	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-expression of syntaxin 1A inhibits cAMP-stimulated current and capacitance changes in CFTR expressing cells and blocks cAMP-induced increases in cell surface CFTR .
	manualset3
245897	1	425337	7	NULL	NULL	0	NULL	Co-infection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-infection of hepatitis C virus ( HCV ) with other blood-borne pathogens such as human T cell leukemia virus ( HTLV ) is common in highly endemic areas .
	manualset3
245898	2	425337	7	NULL	NULL	0	NULL	hepatitis C virus ( HCV )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-infection of hepatitis C virus ( HCV ) with other blood-borne pathogens such as human T cell leukemia virus ( HTLV ) is common in highly endemic areas .
	manualset3
245899	3	425337	7	NULL	NULL	0	NULL	blood-borne pathogens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-infection of hepatitis C virus ( HCV ) with other blood-borne pathogens such as human T cell leukemia virus ( HTLV ) is common in highly endemic areas .
	manualset3
245900	4	425337	7	NULL	NULL	0	NULL	human T cell leukemia virus ( HTLV )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-infection of hepatitis C virus ( HCV ) with other blood-borne pathogens such as human T cell leukemia virus ( HTLV ) is common in highly endemic areas .
	manualset3
245901	5	425337	7	NULL	NULL	0	NULL	highly endemic areas	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-infection of hepatitis C virus ( HCV ) with other blood-borne pathogens such as human T cell leukemia virus ( HTLV ) is common in highly endemic areas .
	manualset3
245902	1	425338	7	NULL	NULL	0	NULL	Co-infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-infection of rAdAAVrep-cap together with rAdAAVGFP into 293 cells resulted in production of high titers of rAAV expressing GFP .
	manualset3
245903	2	425338	7	NULL	NULL	0	NULL	 rAdAAVrep-cap	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-infection of rAdAAVrep-cap together with rAdAAVGFP into 293 cells resulted in production of high titers of rAAV expressing GFP .
	manualset3
245904	3	425338	7	NULL	NULL	0	NULL	rAdAAVGFP	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-infection of rAdAAVrep-cap together with rAdAAVGFP into 293 cells resulted in production of high titers of rAAV expressing GFP .
	manualset3
245905	4	425338	7	NULL	NULL	0	NULL	293 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-infection of rAdAAVrep-cap together with rAdAAVGFP into 293 cells resulted in production of high titers of rAAV expressing GFP .
	manualset3
245906	5	425338	7	NULL	NULL	0	NULL	production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-infection of rAdAAVrep-cap together with rAdAAVGFP into 293 cells resulted in production of high titers of rAAV expressing GFP .
	manualset3
245907	6	425338	7	NULL	NULL	0	NULL	high titers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-infection of rAdAAVrep-cap together with rAdAAVGFP into 293 cells resulted in production of high titers of rAAV expressing GFP .
	manualset3
245908	7	425338	7	NULL	NULL	0	NULL	rAAV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-infection of rAdAAVrep-cap together with rAdAAVGFP into 293 cells resulted in production of high titers of rAAV expressing GFP .
	manualset3
245909	8	425338	7	NULL	NULL	0	NULL	GFP 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-infection of rAdAAVrep-cap together with rAdAAVGFP into 293 cells resulted in production of high titers of rAAV expressing GFP .
	manualset3
245910	1	425339	7	NULL	NULL	0	NULL	Co-operation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-operation between the Institute of Public Health for North Rhine Westphalia , the local health authority of the Hoexter district and the Institute for Geoinformatics of the University of Muenster started a project testing the use of GIS for drinking water surveillance .
	manualset3
245911	2	425339	7	NULL	NULL	0	NULL	Institute of Public Health	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-operation between the Institute of Public Health for North Rhine Westphalia , the local health authority of the Hoexter district and the Institute for Geoinformatics of the University of Muenster started a project testing the use of GIS for drinking water surveillance .
	manualset3
245912	3	425339	7	NULL	NULL	0	NULL	North Rhine Westphalia	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-operation between the Institute of Public Health for North Rhine Westphalia , the local health authority of the Hoexter district and the Institute for Geoinformatics of the University of Muenster started a project testing the use of GIS for drinking water surveillance .
	manualset3
245913	4	425339	7	NULL	NULL	0	NULL	 local health authority	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-operation between the Institute of Public Health for North Rhine Westphalia , the local health authority of the Hoexter district and the Institute for Geoinformatics of the University of Muenster started a project testing the use of GIS for drinking water surveillance .
	manualset3
245914	5	425339	7	NULL	NULL	0	NULL	Hoexter district	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-operation between the Institute of Public Health for North Rhine Westphalia , the local health authority of the Hoexter district and the Institute for Geoinformatics of the University of Muenster started a project testing the use of GIS for drinking water surveillance .
	manualset3
245915	6	425339	7	NULL	NULL	0	NULL	Institute for Geoinformatics 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-operation between the Institute of Public Health for North Rhine Westphalia , the local health authority of the Hoexter district and the Institute for Geoinformatics of the University of Muenster started a project testing the use of GIS for drinking water surveillance .
	manualset3
245916	7	425339	7	NULL	NULL	0	NULL	University of Muenster	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-operation between the Institute of Public Health for North Rhine Westphalia , the local health authority of the Hoexter district and the Institute for Geoinformatics of the University of Muenster started a project testing the use of GIS for drinking water surveillance .
	manualset3
245917	8	425339	7	NULL	NULL	0	NULL	project testing 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-operation between the Institute of Public Health for North Rhine Westphalia , the local health authority of the Hoexter district and the Institute for Geoinformatics of the University of Muenster started a project testing the use of GIS for drinking water surveillance .
	manualset3
245918	9	425339	7	NULL	NULL	0	NULL	 use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-operation between the Institute of Public Health for North Rhine Westphalia , the local health authority of the Hoexter district and the Institute for Geoinformatics of the University of Muenster started a project testing the use of GIS for drinking water surveillance .
	manualset3
245919	10	425339	7	NULL	NULL	0	NULL	GIS	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-operation between the Institute of Public Health for North Rhine Westphalia , the local health authority of the Hoexter district and the Institute for Geoinformatics of the University of Muenster started a project testing the use of GIS for drinking water surveillance .
	manualset3
245920	11	425339	7	NULL	NULL	0	NULL	drinking water surveillance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-operation between the Institute of Public Health for North Rhine Westphalia , the local health authority of the Hoexter district and the Institute for Geoinformatics of the University of Muenster started a project testing the use of GIS for drinking water surveillance .
	manualset3
245921	1	425340	7	NULL	NULL	0	NULL	Co-sleeping	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-sleeping ( sleeping with a parent or sibling ) was noted more frequently in sleep-disturbed ( 34 % ) than in non-sleep-disturbed ( 16 % ) children .
	manualset3
245922	2	425340	7	NULL	NULL	0	NULL	sleeping	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-sleeping ( sleeping with a parent or sibling ) was noted more frequently in sleep-disturbed ( 34 % ) than in non-sleep-disturbed ( 16 % ) children .
	manualset3
245923	3	425340	7	NULL	NULL	0	NULL	parent 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-sleeping ( sleeping with a parent or sibling ) was noted more frequently in sleep-disturbed ( 34 % ) than in non-sleep-disturbed ( 16 % ) children .
	manualset3
245924	4	425340	7	NULL	NULL	0	NULL	sibling	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-sleeping ( sleeping with a parent or sibling ) was noted more frequently in sleep-disturbed ( 34 % ) than in non-sleep-disturbed ( 16 % ) children .
	manualset3
245925	5	425340	7	NULL	NULL	0	NULL	 sleep-disturbed children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-sleeping ( sleeping with a parent or sibling ) was noted more frequently in sleep-disturbed ( 34 % ) than in non-sleep-disturbed ( 16 % ) children .
	manualset3
245926	6	425340	7	NULL	NULL	0	NULL	34 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-sleeping ( sleeping with a parent or sibling ) was noted more frequently in sleep-disturbed ( 34 % ) than in non-sleep-disturbed ( 16 % ) children .
	manualset3
245927	7	425340	7	NULL	NULL	0	NULL	non-sleep-disturbed children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-sleeping ( sleeping with a parent or sibling ) was noted more frequently in sleep-disturbed ( 34 % ) than in non-sleep-disturbed ( 16 % ) children .
	manualset3
245928	8	425340	7	NULL	NULL	0	NULL	16 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-sleeping ( sleeping with a parent or sibling ) was noted more frequently in sleep-disturbed ( 34 % ) than in non-sleep-disturbed ( 16 % ) children .
	manualset3
245929	1	425341	7	NULL	NULL	0	NULL	Intertriginous vesicle development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intertriginous vesicle and pustule development in a 36-year old ) .
	manualset3
245930	2	425341	7	NULL	NULL	0	NULL	pustule development 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intertriginous vesicle and pustule development in a 36-year old ) .
	manualset3
245931	3	425341	7	NULL	NULL	0	NULL	36-year old 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intertriginous vesicle and pustule development in a 36-year old ) .
	manualset3
245932	1	425342	7	NULL	NULL	0	NULL	Co-treatment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-treatment with VER reduced the severity of microcalcification in CsA groups , particularly N animals , increased CCR on day 14 in the Sl ( 196 + / - 23 vs 391 + / - 64 ) and days 21 and 28 in N ( 141 + / - 14 vs 357 + / - 32 and 152 + / - 28 vs 261 + / - 20 ) groups , respectively but had no effect on the magnitude of enzymuria , despite significantly increased trough whole blood CsA levels ( 20-30 % ) in both Sl and N groups .
	manualset3
245933	2	425342	7	NULL	NULL	0	NULL	VER	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-treatment with VER reduced the severity of microcalcification in CsA groups , particularly N animals , increased CCR on day 14 in the Sl ( 196 + / - 23 vs 391 + / - 64 ) and days 21 and 28 in N ( 141 + / - 14 vs 357 + / - 32 and 152 + / - 28 vs 261 + / - 20 ) groups , respectively but had no effect on the magnitude of enzymuria , despite significantly increased trough whole blood CsA levels ( 20-30 % ) in both Sl and N groups .
	manualset3
245934	3	425342	7	NULL	NULL	0	NULL	severity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-treatment with VER reduced the severity of microcalcification in CsA groups , particularly N animals , increased CCR on day 14 in the Sl ( 196 + / - 23 vs 391 + / - 64 ) and days 21 and 28 in N ( 141 + / - 14 vs 357 + / - 32 and 152 + / - 28 vs 261 + / - 20 ) groups , respectively but had no effect on the magnitude of enzymuria , despite significantly increased trough whole blood CsA levels ( 20-30 % ) in both Sl and N groups .
	manualset3
245935	4	425342	7	NULL	NULL	0	NULL	microcalcification	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-treatment with VER reduced the severity of microcalcification in CsA groups , particularly N animals , increased CCR on day 14 in the Sl ( 196 + / - 23 vs 391 + / - 64 ) and days 21 and 28 in N ( 141 + / - 14 vs 357 + / - 32 and 152 + / - 28 vs 261 + / - 20 ) groups , respectively but had no effect on the magnitude of enzymuria , despite significantly increased trough whole blood CsA levels ( 20-30 % ) in both Sl and N groups .
	manualset3
245936	5	425342	7	NULL	NULL	0	NULL	CsA groups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-treatment with VER reduced the severity of microcalcification in CsA groups , particularly N animals , increased CCR on day 14 in the Sl ( 196 + / - 23 vs 391 + / - 64 ) and days 21 and 28 in N ( 141 + / - 14 vs 357 + / - 32 and 152 + / - 28 vs 261 + / - 20 ) groups , respectively but had no effect on the magnitude of enzymuria , despite significantly increased trough whole blood CsA levels ( 20-30 % ) in both Sl and N groups .
	manualset3
245937	6	425342	7	NULL	NULL	0	NULL	N animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-treatment with VER reduced the severity of microcalcification in CsA groups , particularly N animals , increased CCR on day 14 in the Sl ( 196 + / - 23 vs 391 + / - 64 ) and days 21 and 28 in N ( 141 + / - 14 vs 357 + / - 32 and 152 + / - 28 vs 261 + / - 20 ) groups , respectively but had no effect on the magnitude of enzymuria , despite significantly increased trough whole blood CsA levels ( 20-30 % ) in both Sl and N groups .
	manualset3
245938	7	425342	7	NULL	NULL	0	NULL	CCR	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-treatment with VER reduced the severity of microcalcification in CsA groups , particularly N animals , increased CCR on day 14 in the Sl ( 196 + / - 23 vs 391 + / - 64 ) and days 21 and 28 in N ( 141 + / - 14 vs 357 + / - 32 and 152 + / - 28 vs 261 + / - 20 ) groups , respectively but had no effect on the magnitude of enzymuria , despite significantly increased trough whole blood CsA levels ( 20-30 % ) in both Sl and N groups .
	manualset3
245939	8	425342	7	NULL	NULL	0	NULL	day 14	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-treatment with VER reduced the severity of microcalcification in CsA groups , particularly N animals , increased CCR on day 14 in the Sl ( 196 + / - 23 vs 391 + / - 64 ) and days 21 and 28 in N ( 141 + / - 14 vs 357 + / - 32 and 152 + / - 28 vs 261 + / - 20 ) groups , respectively but had no effect on the magnitude of enzymuria , despite significantly increased trough whole blood CsA levels ( 20-30 % ) in both Sl and N groups .
	manualset3
245940	9	425342	7	NULL	NULL	0	NULL	SI	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-treatment with VER reduced the severity of microcalcification in CsA groups , particularly N animals , increased CCR on day 14 in the Sl ( 196 + / - 23 vs 391 + / - 64 ) and days 21 and 28 in N ( 141 + / - 14 vs 357 + / - 32 and 152 + / - 28 vs 261 + / - 20 ) groups , respectively but had no effect on the magnitude of enzymuria , despite significantly increased trough whole blood CsA levels ( 20-30 % ) in both Sl and N groups .
	manualset3
245941	10	425342	7	NULL	NULL	0	NULL	196 + / - 23	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-treatment with VER reduced the severity of microcalcification in CsA groups , particularly N animals , increased CCR on day 14 in the Sl ( 196 + / - 23 vs 391 + / - 64 ) and days 21 and 28 in N ( 141 + / - 14 vs 357 + / - 32 and 152 + / - 28 vs 261 + / - 20 ) groups , respectively but had no effect on the magnitude of enzymuria , despite significantly increased trough whole blood CsA levels ( 20-30 % ) in both Sl and N groups .
	manualset3
245942	11	425342	7	NULL	NULL	0	NULL	391 + / - 64	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-treatment with VER reduced the severity of microcalcification in CsA groups , particularly N animals , increased CCR on day 14 in the Sl ( 196 + / - 23 vs 391 + / - 64 ) and days 21 and 28 in N ( 141 + / - 14 vs 357 + / - 32 and 152 + / - 28 vs 261 + / - 20 ) groups , respectively but had no effect on the magnitude of enzymuria , despite significantly increased trough whole blood CsA levels ( 20-30 % ) in both Sl and N groups .
	manualset3
245943	12	425342	7	NULL	NULL	0	NULL	days 21	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-treatment with VER reduced the severity of microcalcification in CsA groups , particularly N animals , increased CCR on day 14 in the Sl ( 196 + / - 23 vs 391 + / - 64 ) and days 21 and 28 in N ( 141 + / - 14 vs 357 + / - 32 and 152 + / - 28 vs 261 + / - 20 ) groups , respectively but had no effect on the magnitude of enzymuria , despite significantly increased trough whole blood CsA levels ( 20-30 % ) in both Sl and N groups .
	manualset3
245944	13	425342	7	NULL	NULL	0	NULL	days 28	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-treatment with VER reduced the severity of microcalcification in CsA groups , particularly N animals , increased CCR on day 14 in the Sl ( 196 + / - 23 vs 391 + / - 64 ) and days 21 and 28 in N ( 141 + / - 14 vs 357 + / - 32 and 152 + / - 28 vs 261 + / - 20 ) groups , respectively but had no effect on the magnitude of enzymuria , despite significantly increased trough whole blood CsA levels ( 20-30 % ) in both Sl and N groups .
	manualset3
245945	14	425342	7	NULL	NULL	0	NULL	N groups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-treatment with VER reduced the severity of microcalcification in CsA groups , particularly N animals , increased CCR on day 14 in the Sl ( 196 + / - 23 vs 391 + / - 64 ) and days 21 and 28 in N ( 141 + / - 14 vs 357 + / - 32 and 152 + / - 28 vs 261 + / - 20 ) groups , respectively but had no effect on the magnitude of enzymuria , despite significantly increased trough whole blood CsA levels ( 20-30 % ) in both Sl and N groups .
	manualset3
245946	15	425342	7	NULL	NULL	0	NULL	141 + / - 14	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-treatment with VER reduced the severity of microcalcification in CsA groups , particularly N animals , increased CCR on day 14 in the Sl ( 196 + / - 23 vs 391 + / - 64 ) and days 21 and 28 in N ( 141 + / - 14 vs 357 + / - 32 and 152 + / - 28 vs 261 + / - 20 ) groups , respectively but had no effect on the magnitude of enzymuria , despite significantly increased trough whole blood CsA levels ( 20-30 % ) in both Sl and N groups .
	manualset3
245947	16	425342	7	NULL	NULL	0	NULL	357 + / - 32	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-treatment with VER reduced the severity of microcalcification in CsA groups , particularly N animals , increased CCR on day 14 in the Sl ( 196 + / - 23 vs 391 + / - 64 ) and days 21 and 28 in N ( 141 + / - 14 vs 357 + / - 32 and 152 + / - 28 vs 261 + / - 20 ) groups , respectively but had no effect on the magnitude of enzymuria , despite significantly increased trough whole blood CsA levels ( 20-30 % ) in both Sl and N groups .
	manualset3
245948	17	425342	7	NULL	NULL	0	NULL	152 + / - 28	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-treatment with VER reduced the severity of microcalcification in CsA groups , particularly N animals , increased CCR on day 14 in the Sl ( 196 + / - 23 vs 391 + / - 64 ) and days 21 and 28 in N ( 141 + / - 14 vs 357 + / - 32 and 152 + / - 28 vs 261 + / - 20 ) groups , respectively but had no effect on the magnitude of enzymuria , despite significantly increased trough whole blood CsA levels ( 20-30 % ) in both Sl and N groups .
	manualset3
245949	18	425342	7	NULL	NULL	0	NULL	 261 + / - 20	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-treatment with VER reduced the severity of microcalcification in CsA groups , particularly N animals , increased CCR on day 14 in the Sl ( 196 + / - 23 vs 391 + / - 64 ) and days 21 and 28 in N ( 141 + / - 14 vs 357 + / - 32 and 152 + / - 28 vs 261 + / - 20 ) groups , respectively but had no effect on the magnitude of enzymuria , despite significantly increased trough whole blood CsA levels ( 20-30 % ) in both Sl and N groups .
	manualset3
245950	19	425342	7	NULL	NULL	0	NULL	no effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-treatment with VER reduced the severity of microcalcification in CsA groups , particularly N animals , increased CCR on day 14 in the Sl ( 196 + / - 23 vs 391 + / - 64 ) and days 21 and 28 in N ( 141 + / - 14 vs 357 + / - 32 and 152 + / - 28 vs 261 + / - 20 ) groups , respectively but had no effect on the magnitude of enzymuria , despite significantly increased trough whole blood CsA levels ( 20-30 % ) in both Sl and N groups .
	manualset3
245951	20	425342	7	NULL	NULL	0	NULL	magnitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-treatment with VER reduced the severity of microcalcification in CsA groups , particularly N animals , increased CCR on day 14 in the Sl ( 196 + / - 23 vs 391 + / - 64 ) and days 21 and 28 in N ( 141 + / - 14 vs 357 + / - 32 and 152 + / - 28 vs 261 + / - 20 ) groups , respectively but had no effect on the magnitude of enzymuria , despite significantly increased trough whole blood CsA levels ( 20-30 % ) in both Sl and N groups .
	manualset3
245952	21	425342	7	NULL	NULL	0	NULL	enzymuria	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-treatment with VER reduced the severity of microcalcification in CsA groups , particularly N animals , increased CCR on day 14 in the Sl ( 196 + / - 23 vs 391 + / - 64 ) and days 21 and 28 in N ( 141 + / - 14 vs 357 + / - 32 and 152 + / - 28 vs 261 + / - 20 ) groups , respectively but had no effect on the magnitude of enzymuria , despite significantly increased trough whole blood CsA levels ( 20-30 % ) in both Sl and N groups .
	manualset3
245953	22	425342	7	NULL	NULL	0	NULL	 whole blood CsA levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-treatment with VER reduced the severity of microcalcification in CsA groups , particularly N animals , increased CCR on day 14 in the Sl ( 196 + / - 23 vs 391 + / - 64 ) and days 21 and 28 in N ( 141 + / - 14 vs 357 + / - 32 and 152 + / - 28 vs 261 + / - 20 ) groups , respectively but had no effect on the magnitude of enzymuria , despite significantly increased trough whole blood CsA levels ( 20-30 % ) in both Sl and N groups .
	manualset3
245954	23	425342	7	NULL	NULL	0	NULL	20-30 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-treatment with VER reduced the severity of microcalcification in CsA groups , particularly N animals , increased CCR on day 14 in the Sl ( 196 + / - 23 vs 391 + / - 64 ) and days 21 and 28 in N ( 141 + / - 14 vs 357 + / - 32 and 152 + / - 28 vs 261 + / - 20 ) groups , respectively but had no effect on the magnitude of enzymuria , despite significantly increased trough whole blood CsA levels ( 20-30 % ) in both Sl and N groups .
	manualset3
245955	24	425342	7	NULL	NULL	0	NULL	Sl groups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-treatment with VER reduced the severity of microcalcification in CsA groups , particularly N animals , increased CCR on day 14 in the Sl ( 196 + / - 23 vs 391 + / - 64 ) and days 21 and 28 in N ( 141 + / - 14 vs 357 + / - 32 and 152 + / - 28 vs 261 + / - 20 ) groups , respectively but had no effect on the magnitude of enzymuria , despite significantly increased trough whole blood CsA levels ( 20-30 % ) in both Sl and N groups .
	manualset3
245956	25	425342	7	NULL	NULL	0	NULL	N groups 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Co-treatment with VER reduced the severity of microcalcification in CsA groups , particularly N animals , increased CCR on day 14 in the Sl ( 196 + / - 23 vs 391 + / - 64 ) and days 21 and 28 in N ( 141 + / - 14 vs 357 + / - 32 and 152 + / - 28 vs 261 + / - 20 ) groups , respectively but had no effect on the magnitude of enzymuria , despite significantly increased trough whole blood CsA levels ( 20-30 % ) in both Sl and N groups .
	manualset3
245957	1	425343	7	NULL	NULL	0	NULL	CoNS strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	CoNS strains ( n = 745 ) isolated from a university teaching hospital in China between 2004 and 2009 were tested for antibiotic resistance .
	manualset3
245958	2	425343	7	NULL	NULL	0	NULL	n = 745	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	CoNS strains ( n = 745 ) isolated from a university teaching hospital in China between 2004 and 2009 were tested for antibiotic resistance .
	manualset3
245959	3	425343	7	NULL	NULL	0	NULL	university teaching hospital 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	CoNS strains ( n = 745 ) isolated from a university teaching hospital in China between 2004 and 2009 were tested for antibiotic resistance .
	manualset3
245960	4	425343	7	NULL	NULL	0	NULL	China	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	CoNS strains ( n = 745 ) isolated from a university teaching hospital in China between 2004 and 2009 were tested for antibiotic resistance .
	manualset3
245961	5	425343	7	NULL	NULL	0	NULL	2004	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	CoNS strains ( n = 745 ) isolated from a university teaching hospital in China between 2004 and 2009 were tested for antibiotic resistance .
	manualset3
245962	6	425343	7	NULL	NULL	0	NULL	2009	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	CoNS strains ( n = 745 ) isolated from a university teaching hospital in China between 2004 and 2009 were tested for antibiotic resistance .
	manualset3
245963	7	425343	7	NULL	NULL	0	NULL	antibiotic resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	CoNS strains ( n = 745 ) isolated from a university teaching hospital in China between 2004 and 2009 were tested for antibiotic resistance .
	manualset3
245964	1	425344	7	NULL	NULL	NULL	NULL	Coactivation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coactivation by OCA-B : definition of critical regions and synergism with general cofactors .
	manualset3
245965	2	425344	7	NULL	NULL	0	NULL	 OCA-B 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Coactivation by OCA-B : definition of critical regions and synergism with general cofactors .
	manualset3
245966	3	425344	7	NULL	NULL	0	NULL	definition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Coactivation by OCA-B : definition of critical regions and synergism with general cofactors .
	manualset3
245967	4	425344	7	NULL	NULL	0	NULL	 critical regions	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Coactivation by OCA-B : definition of critical regions and synergism with general cofactors .
	manualset3
245968	5	425344	7	NULL	NULL	0	NULL	synergism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Coactivation by OCA-B : definition of critical regions and synergism with general cofactors .
	manualset3
245969	6	425344	7	NULL	NULL	0	NULL	cofactors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Coactivation by OCA-B : definition of critical regions and synergism with general cofactors .
	manualset3
245970	1	425345	7	NULL	NULL	0	NULL	Coagulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulation and the changing value of the coagulation factor were regularly measured , and 70 % of the normal value of coagulation factor IX was maintained through the injection of recombinant coagulation factors and antihemorrhagics .
	manualset3
245971	2	425345	7	NULL	NULL	0	NULL	changing value 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulation and the changing value of the coagulation factor were regularly measured , and 70 % of the normal value of coagulation factor IX was maintained through the injection of recombinant coagulation factors and antihemorrhagics .
	manualset3
245972	3	425345	7	NULL	NULL	0	NULL	coagulation factor	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulation and the changing value of the coagulation factor were regularly measured , and 70 % of the normal value of coagulation factor IX was maintained through the injection of recombinant coagulation factors and antihemorrhagics .
	manualset3
245973	4	425345	7	NULL	NULL	0	NULL	 70 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulation and the changing value of the coagulation factor were regularly measured , and 70 % of the normal value of coagulation factor IX was maintained through the injection of recombinant coagulation factors and antihemorrhagics .
	manualset3
245974	5	425345	7	NULL	NULL	0	NULL	normal value	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulation and the changing value of the coagulation factor were regularly measured , and 70 % of the normal value of coagulation factor IX was maintained through the injection of recombinant coagulation factors and antihemorrhagics .
	manualset3
245975	6	425345	7	NULL	NULL	0	NULL	coagulation factor IX	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulation and the changing value of the coagulation factor were regularly measured , and 70 % of the normal value of coagulation factor IX was maintained through the injection of recombinant coagulation factors and antihemorrhagics .
	manualset3
245976	7	425345	7	NULL	NULL	0	NULL	injection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulation and the changing value of the coagulation factor were regularly measured , and 70 % of the normal value of coagulation factor IX was maintained through the injection of recombinant coagulation factors and antihemorrhagics .
	manualset3
245977	8	425345	7	NULL	NULL	0	NULL	recombinant coagulation factors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulation and the changing value of the coagulation factor were regularly measured , and 70 % of the normal value of coagulation factor IX was maintained through the injection of recombinant coagulation factors and antihemorrhagics .
	manualset3
245978	9	425345	7	NULL	NULL	0	NULL	antihemorrhagics 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulation and the changing value of the coagulation factor were regularly measured , and 70 % of the normal value of coagulation factor IX was maintained through the injection of recombinant coagulation factors and antihemorrhagics .
	manualset3
245979	1	425346	7	NULL	NULL	0	NULL	Coagulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulation in the secondary energy minimum can only explain the aggregation efficiency of topsoil colloids at low Ca ( 2 + ) concentrations ( & lt ; 2 mM Ca ( 2 + ) ) under unfavorable electrostatic conditions .
	manualset3
245980	2	425346	7	NULL	NULL	0	NULL	secondary energy minimum	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulation in the secondary energy minimum can only explain the aggregation efficiency of topsoil colloids at low Ca ( 2 + ) concentrations ( & lt ; 2 mM Ca ( 2 + ) ) under unfavorable electrostatic conditions .
	manualset3
245981	3	425346	7	NULL	NULL	0	NULL	aggregation efficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulation in the secondary energy minimum can only explain the aggregation efficiency of topsoil colloids at low Ca ( 2 + ) concentrations ( & lt ; 2 mM Ca ( 2 + ) ) under unfavorable electrostatic conditions .
	manualset3
245982	4	425346	7	NULL	NULL	0	NULL	topsoil colloids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulation in the secondary energy minimum can only explain the aggregation efficiency of topsoil colloids at low Ca ( 2 + ) concentrations ( & lt ; 2 mM Ca ( 2 + ) ) under unfavorable electrostatic conditions .
	manualset3
245983	5	425346	7	NULL	NULL	0	NULL	low Ca ( 2 + ) concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulation in the secondary energy minimum can only explain the aggregation efficiency of topsoil colloids at low Ca ( 2 + ) concentrations ( & lt ; 2 mM Ca ( 2 + ) ) under unfavorable electrostatic conditions .
	manualset3
245984	6	425346	7	NULL	NULL	0	NULL	& lt	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulation in the secondary energy minimum can only explain the aggregation efficiency of topsoil colloids at low Ca ( 2 + ) concentrations ( & lt ; 2 mM Ca ( 2 + ) ) under unfavorable electrostatic conditions .
	manualset3
245985	7	425346	7	NULL	NULL	0	NULL	2 mM Ca ( 2 + )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulation in the secondary energy minimum can only explain the aggregation efficiency of topsoil colloids at low Ca ( 2 + ) concentrations ( & lt ; 2 mM Ca ( 2 + ) ) under unfavorable electrostatic conditions .
	manualset3
245986	8	425346	7	NULL	NULL	0	NULL	unfavorable electrostatic conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulation in the secondary energy minimum can only explain the aggregation efficiency of topsoil colloids at low Ca ( 2 + ) concentrations ( & lt ; 2 mM Ca ( 2 + ) ) under unfavorable electrostatic conditions .
	manualset3
245987	1	425347	7	NULL	NULL	0	NULL	Coagulation parameters	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulation parameters ( fibrinogen concentration , thrombin time , PT and aPTT ) and hematological parameters remained normal over the course of the study when compared to initial values of the subject swine .
	manualset3
245988	2	425347	7	NULL	NULL	0	NULL	 fibrinogen concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulation parameters ( fibrinogen concentration , thrombin time , PT and aPTT ) and hematological parameters remained normal over the course of the study when compared to initial values of the subject swine .
	manualset3
245989	3	425347	7	NULL	NULL	0	NULL	thrombin time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulation parameters ( fibrinogen concentration , thrombin time , PT and aPTT ) and hematological parameters remained normal over the course of the study when compared to initial values of the subject swine .
	manualset3
245990	4	425347	7	NULL	NULL	0	NULL	 PT	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulation parameters ( fibrinogen concentration , thrombin time , PT and aPTT ) and hematological parameters remained normal over the course of the study when compared to initial values of the subject swine .
	manualset3
245991	5	425347	7	NULL	NULL	0	NULL	PTT	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulation parameters ( fibrinogen concentration , thrombin time , PT and aPTT ) and hematological parameters remained normal over the course of the study when compared to initial values of the subject swine .
	manualset3
245992	6	425347	7	NULL	NULL	0	NULL	hematological parameters	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulation parameters ( fibrinogen concentration , thrombin time , PT and aPTT ) and hematological parameters remained normal over the course of the study when compared to initial values of the subject swine .
	manualset3
245993	7	425347	7	NULL	NULL	0	NULL	course	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulation parameters ( fibrinogen concentration , thrombin time , PT and aPTT ) and hematological parameters remained normal over the course of the study when compared to initial values of the subject swine .
	manualset3
245994	8	425347	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulation parameters ( fibrinogen concentration , thrombin time , PT and aPTT ) and hematological parameters remained normal over the course of the study when compared to initial values of the subject swine .
	manualset3
245995	9	425347	7	NULL	NULL	0	NULL	 initial values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulation parameters ( fibrinogen concentration , thrombin time , PT and aPTT ) and hematological parameters remained normal over the course of the study when compared to initial values of the subject swine .
	manualset3
245996	10	425347	7	NULL	NULL	0	NULL	subject swine	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Coagulation parameters ( fibrinogen concentration , thrombin time , PT and aPTT ) and hematological parameters remained normal over the course of the study when compared to initial values of the subject swine .
	manualset3
245997	1	425348	7	NULL	NULL	0	NULL	Coating strategies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Coating strategies based on chemisorption and ligand exchange often provide a better way to tailor the surface properties of NPs .
	manualset3
245998	2	425348	7	NULL	NULL	NULL	NULL	chemisorption 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coating strategies based on chemisorption and ligand exchange often provide a better way to tailor the surface properties of NPs .
	manualset3
245999	3	425348	7	NULL	NULL	0	NULL	 ligand exchange	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Coating strategies based on chemisorption and ligand exchange often provide a better way to tailor the surface properties of NPs .
	manualset3
246000	4	425348	7	NULL	NULL	0	NULL	surface properties 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Coating strategies based on chemisorption and ligand exchange often provide a better way to tailor the surface properties of NPs .
	manualset3
246001	5	425348	7	NULL	NULL	0	NULL	NPs	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Coating strategies based on chemisorption and ligand exchange often provide a better way to tailor the surface properties of NPs .
	manualset3
246002	1	425349	7	NULL	NULL	0	NULL	Cobalt complex	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Cobalt complex with GnRH stimulates the LH release and PKA signaling pathway in pig anterior pituitary cells in vitro .
	manualset3
246003	2	425349	7	NULL	NULL	0	NULL	GnRH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Cobalt complex with GnRH stimulates the LH release and PKA signaling pathway in pig anterior pituitary cells in vitro .
	manualset3
246004	3	425349	7	NULL	NULL	0	NULL	LH release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cobalt complex with GnRH stimulates the LH release and PKA signaling pathway in pig anterior pituitary cells in vitro .
	manualset3
246005	4	425349	7	NULL	NULL	0	NULL	PKA signaling pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cobalt complex with GnRH stimulates the LH release and PKA signaling pathway in pig anterior pituitary cells in vitro .
	manualset3
246006	5	425349	7	NULL	NULL	0	NULL	 pig anterior pituitary cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Cobalt complex with GnRH stimulates the LH release and PKA signaling pathway in pig anterior pituitary cells in vitro .
	manualset3
246007	1	425350	7	NULL	NULL	0	NULL	Cochlear implants	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Cochlear implants in deaf children .
	manualset3
246008	2	425350	7	NULL	NULL	0	NULL	deaf children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Cochlear implants in deaf children .
	manualset3
246009	1	425351	7	NULL	NULL	0	NULL	Intestinal occlusion	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intestinal occlusion caused by retroperitoneal cysts of wolffian origin ) .
	manualset3
246010	2	425351	7	NULL	NULL	0	NULL	retroperitoneal cysts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intestinal occlusion caused by retroperitoneal cysts of wolffian origin ) .
	manualset3
246011	3	425351	7	NULL	NULL	0	NULL	wolffian origin	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intestinal occlusion caused by retroperitoneal cysts of wolffian origin ) .
	manualset3
246012	1	425352	7	NULL	NULL	0	NULL	Coexistence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Coexistence of renal cell carcinoma and renal angiomyolipoma developing in a kidney : a case report .
	manualset3
246013	2	425352	7	NULL	NULL	0	NULL	renal cell carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Coexistence of renal cell carcinoma and renal angiomyolipoma developing in a kidney : a case report .
	manualset3
246014	3	425352	7	NULL	NULL	0	NULL	renal angiomyolipoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Coexistence of renal cell carcinoma and renal angiomyolipoma developing in a kidney : a case report .
	manualset3
246015	4	425352	7	NULL	NULL	0	NULL	 kidney 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Coexistence of renal cell carcinoma and renal angiomyolipoma developing in a kidney : a case report .
	manualset3
246016	5	425352	7	NULL	NULL	0	NULL	case report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Coexistence of renal cell carcinoma and renal angiomyolipoma developing in a kidney : a case report .
	manualset3
246017	1	425353	7	NULL	NULL	0	NULL	ocular myasthenia gravis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Coexistent isolated ocular myasthenia gravis and Graves ' ophthalmopathy is rare and should be considered in patients with findings of ocular myasthenia and extraocular muscle dysfunction .
	manualset3
246018	2	425353	7	NULL	NULL	0	NULL	 Graves ' ophthalmopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Coexistent isolated ocular myasthenia gravis and Graves ' ophthalmopathy is rare and should be considered in patients with findings of ocular myasthenia and extraocular muscle dysfunction .
	manualset3
246019	3	425353	7	NULL	NULL	0	NULL	 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Coexistent isolated ocular myasthenia gravis and Graves ' ophthalmopathy is rare and should be considered in patients with findings of ocular myasthenia and extraocular muscle dysfunction .
	manualset3
246020	4	425353	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Coexistent isolated ocular myasthenia gravis and Graves ' ophthalmopathy is rare and should be considered in patients with findings of ocular myasthenia and extraocular muscle dysfunction .
	manualset3
246021	5	425353	7	NULL	NULL	0	NULL	 ocular myasthenia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Coexistent isolated ocular myasthenia gravis and Graves ' ophthalmopathy is rare and should be considered in patients with findings of ocular myasthenia and extraocular muscle dysfunction .
	manualset3
246022	6	425353	7	NULL	NULL	0	NULL	extraocular muscle dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Coexistent isolated ocular myasthenia gravis and Graves ' ophthalmopathy is rare and should be considered in patients with findings of ocular myasthenia and extraocular muscle dysfunction .
	manualset3
246023	1	425354	7	NULL	NULL	0	NULL	Coexpression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Coexpression of EBV gH and gL facilitated transport of gH to the cell surface and resulted in formation of a stable complex of gH and gL .
	manualset3
246024	2	425354	7	NULL	NULL	0	NULL	EBV gH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Coexpression of EBV gH and gL facilitated transport of gH to the cell surface and resulted in formation of a stable complex of gH and gL .
	manualset3
246025	3	425354	7	NULL	NULL	0	NULL	gL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Coexpression of EBV gH and gL facilitated transport of gH to the cell surface and resulted in formation of a stable complex of gH and gL .
	manualset3
246026	4	425354	7	NULL	NULL	0	NULL	transport 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Coexpression of EBV gH and gL facilitated transport of gH to the cell surface and resulted in formation of a stable complex of gH and gL .
	manualset3
246027	5	425354	7	NULL	NULL	0	NULL	gH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Coexpression of EBV gH and gL facilitated transport of gH to the cell surface and resulted in formation of a stable complex of gH and gL .
	manualset3
246028	6	425354	7	NULL	NULL	0	NULL	cell surface	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Coexpression of EBV gH and gL facilitated transport of gH to the cell surface and resulted in formation of a stable complex of gH and gL .
	manualset3
246029	7	425354	7	NULL	NULL	0	NULL	formation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Coexpression of EBV gH and gL facilitated transport of gH to the cell surface and resulted in formation of a stable complex of gH and gL .
	manualset3
246030	8	425354	7	NULL	NULL	0	NULL	stable complex 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Coexpression of EBV gH and gL facilitated transport of gH to the cell surface and resulted in formation of a stable complex of gH and gL .
	manualset3
246031	9	425354	7	NULL	NULL	0	NULL	gH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Coexpression of EBV gH and gL facilitated transport of gH to the cell surface and resulted in formation of a stable complex of gH and gL .
	manualset3
246032	10	425354	7	NULL	NULL	0	NULL	gL	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Coexpression of EBV gH and gL facilitated transport of gH to the cell surface and resulted in formation of a stable complex of gH and gL .
	manualset3
246033	1	425355	7	NULL	NULL	0	NULL	Coexpression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Coexpression of cholecystokinin-B/gastrin receptor and gastrin gene in human gastric tissues and gastric cancer cell line .
	manualset3
246034	2	425355	7	NULL	NULL	NULL	NULL	cholecystokinin-B/gastrin receptor	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coexpression of cholecystokinin-B/gastrin receptor and gastrin gene in human gastric tissues and gastric cancer cell line .
	manualset3
246035	3	425355	7	NULL	NULL	0	NULL	gastrin gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Coexpression of cholecystokinin-B/gastrin receptor and gastrin gene in human gastric tissues and gastric cancer cell line .
	manualset3
246036	4	425355	7	NULL	NULL	0	NULL	human gastric tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Coexpression of cholecystokinin-B/gastrin receptor and gastrin gene in human gastric tissues and gastric cancer cell line .
	manualset3
246037	5	425355	7	NULL	NULL	0	NULL	gastric cancer cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Coexpression of cholecystokinin-B/gastrin receptor and gastrin gene in human gastric tissues and gastric cancer cell line .
	manualset3
246038	1	425356	7	NULL	NULL	0	NULL	Cognitive brain functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cognitive brain functions , for example , sensory perception , motor control and learning , are understood as computation by axonal-dendritic chemical synapses in networks of integrate-and-fire neurons .
	manualset3
246039	2	425356	7	NULL	NULL	0	NULL	sensory perception	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cognitive brain functions , for example , sensory perception , motor control and learning , are understood as computation by axonal-dendritic chemical synapses in networks of integrate-and-fire neurons .
	manualset3
246040	3	425356	7	NULL	NULL	0	NULL	motor control	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cognitive brain functions , for example , sensory perception , motor control and learning , are understood as computation by axonal-dendritic chemical synapses in networks of integrate-and-fire neurons .
	manualset3
246041	4	425356	7	NULL	NULL	0	NULL	 learning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cognitive brain functions , for example , sensory perception , motor control and learning , are understood as computation by axonal-dendritic chemical synapses in networks of integrate-and-fire neurons .
	manualset3
246042	5	425356	7	NULL	NULL	0	NULL	computation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Cognitive brain functions , for example , sensory perception , motor control and learning , are understood as computation by axonal-dendritic chemical synapses in networks of integrate-and-fire neurons .
	manualset3
246043	6	425356	7	NULL	NULL	NULL	NULL	axonal-dendritic chemical synapses	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cognitive brain functions , for example , sensory perception , motor control and learning , are understood as computation by axonal-dendritic chemical synapses in networks of integrate-and-fire neurons .
	manualset3
246044	7	425356	7	NULL	NULL	0	NULL	networks	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cognitive brain functions , for example , sensory perception , motor control and learning , are understood as computation by axonal-dendritic chemical synapses in networks of integrate-and-fire neurons .
	manualset3
246045	8	425356	7	NULL	NULL	0	NULL	integrate-and-fire neurons 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Cognitive brain functions , for example , sensory perception , motor control and learning , are understood as computation by axonal-dendritic chemical synapses in networks of integrate-and-fire neurons .
	manualset3
246046	9	425356	7	NULL	NULL	0	NULL	example	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Cognitive brain functions , for example , sensory perception , motor control and learning , are understood as computation by axonal-dendritic chemical synapses in networks of integrate-and-fire neurons .
	manualset3
246047	1	425357	7	NULL	NULL	0	NULL	Cognitive functions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cognitive functions were significantly and diffusely impaired in PD when compared with controls who were matched for age as well as for the degree and location of CHs .
	manualset3
246048	2	425357	7	NULL	NULL	0	NULL	PD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Cognitive functions were significantly and diffusely impaired in PD when compared with controls who were matched for age as well as for the degree and location of CHs .
	manualset3
246049	3	425357	7	NULL	NULL	0	NULL	controls 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Cognitive functions were significantly and diffusely impaired in PD when compared with controls who were matched for age as well as for the degree and location of CHs .
	manualset3
246050	4	425357	7	NULL	NULL	0	NULL	age	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cognitive functions were significantly and diffusely impaired in PD when compared with controls who were matched for age as well as for the degree and location of CHs .
	manualset3
246051	5	425357	7	NULL	NULL	0	NULL	degree	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Cognitive functions were significantly and diffusely impaired in PD when compared with controls who were matched for age as well as for the degree and location of CHs .
	manualset3
246052	6	425357	7	NULL	NULL	0	NULL	location	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Cognitive functions were significantly and diffusely impaired in PD when compared with controls who were matched for age as well as for the degree and location of CHs .
	manualset3
246053	7	425357	7	NULL	NULL	0	NULL	CHs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Cognitive functions were significantly and diffusely impaired in PD when compared with controls who were matched for age as well as for the degree and location of CHs .
	manualset3
246054	1	425358	7	NULL	NULL	0	NULL	investigation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Coincident to this investigation , we used reverse-transcription polymerase chain reaction techniques to analyze the effects of chronic ( ) propranolol on markers of striatal activity known to be involved in LID .
	manualset3
246055	2	425358	7	NULL	NULL	0	NULL	reverse-transcription polymerase chain reaction techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Coincident to this investigation , we used reverse-transcription polymerase chain reaction techniques to analyze the effects of chronic ( ) propranolol on markers of striatal activity known to be involved in LID .
	manualset3
246056	3	425358	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Coincident to this investigation , we used reverse-transcription polymerase chain reaction techniques to analyze the effects of chronic ( ) propranolol on markers of striatal activity known to be involved in LID .
	manualset3
246057	4	425358	7	NULL	NULL	0	NULL	chronic ( ) propranolol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Coincident to this investigation , we used reverse-transcription polymerase chain reaction techniques to analyze the effects of chronic ( ) propranolol on markers of striatal activity known to be involved in LID .
	manualset3
246058	5	425358	7	NULL	NULL	0	NULL	markers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Coincident to this investigation , we used reverse-transcription polymerase chain reaction techniques to analyze the effects of chronic ( ) propranolol on markers of striatal activity known to be involved in LID .
	manualset3
246059	6	425358	7	NULL	NULL	0	NULL	striatal activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Coincident to this investigation , we used reverse-transcription polymerase chain reaction techniques to analyze the effects of chronic ( ) propranolol on markers of striatal activity known to be involved in LID .
	manualset3
246060	7	425358	7	NULL	NULL	0	NULL	LID	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Coincident to this investigation , we used reverse-transcription polymerase chain reaction techniques to analyze the effects of chronic ( ) propranolol on markers of striatal activity known to be involved in LID .
	manualset3
246061	1	425359	7	NULL	NULL	0	NULL	Intra-arterial use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intra-arterial use of microencapsulated mitomycin C in the treatment of advanced carcinoma ( author 's transl ) ) .
	manualset3
246062	2	425359	7	NULL	NULL	0	NULL	microencapsulated mitomycin C	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intra-arterial use of microencapsulated mitomycin C in the treatment of advanced carcinoma ( author 's transl ) ) .
	manualset3
246063	3	425359	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intra-arterial use of microencapsulated mitomycin C in the treatment of advanced carcinoma ( author 's transl ) ) .
	manualset3
246064	4	425359	7	NULL	NULL	0	NULL	advanced carcinoma 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intra-arterial use of microencapsulated mitomycin C in the treatment of advanced carcinoma ( author 's transl ) ) .
	manualset3
246065	5	425359	7	NULL	NULL	0	NULL	author 's transl	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intra-arterial use of microencapsulated mitomycin C in the treatment of advanced carcinoma ( author 's transl ) ) .
	manualset3
246066	1	425360	7	NULL	NULL	0	NULL	Colchicine-induced Mallory body formation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Colchicine-induced Mallory body formation in the mouse .
	manualset3
246067	2	425360	7	NULL	NULL	0	NULL	mouse	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Colchicine-induced Mallory body formation in the mouse .
	manualset3
246068	1	425361	7	NULL	NULL	0	NULL	Cold-insoluble globulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Cold-insoluble globulin mediates the adhesion of rat liver cells to plastic Petri dishes .
	manualset3
246069	2	425361	7	NULL	NULL	0	NULL	adhesion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Cold-insoluble globulin mediates the adhesion of rat liver cells to plastic Petri dishes .
	manualset3
246070	3	425361	7	NULL	NULL	0	NULL	rat liver cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Cold-insoluble globulin mediates the adhesion of rat liver cells to plastic Petri dishes .
	manualset3
246071	4	425361	7	NULL	NULL	0	NULL	plastic Petri dishes	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Cold-insoluble globulin mediates the adhesion of rat liver cells to plastic Petri dishes .
	manualset3
246072	1	425362	7	NULL	NULL	0	NULL	Colitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Colitis was induced in rats with intracolonic 2 , 4 , 6-trinitrobenzenesulfonic acid ( TNBS , 30 mg ) in 50 % ethanol .
	manualset3
246073	2	425362	7	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Colitis was induced in rats with intracolonic 2 , 4 , 6-trinitrobenzenesulfonic acid ( TNBS , 30 mg ) in 50 % ethanol .
	manualset3
246074	3	425362	7	NULL	NULL	0	NULL	intracolonic 2 , 4 , 6-trinitrobenzenesulfonic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Colitis was induced in rats with intracolonic 2 , 4 , 6-trinitrobenzenesulfonic acid ( TNBS , 30 mg ) in 50 % ethanol .
	manualset3
246075	4	425362	7	NULL	NULL	0	NULL	TNBS	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Colitis was induced in rats with intracolonic 2 , 4 , 6-trinitrobenzenesulfonic acid ( TNBS , 30 mg ) in 50 % ethanol .
	manualset3
246076	5	425362	7	NULL	NULL	0	NULL	30 mg	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Colitis was induced in rats with intracolonic 2 , 4 , 6-trinitrobenzenesulfonic acid ( TNBS , 30 mg ) in 50 % ethanol .
	manualset3
246077	6	425362	7	NULL	NULL	NULL	NULL	50 % 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Colitis was induced in rats with intracolonic 2 , 4 , 6-trinitrobenzenesulfonic acid ( TNBS , 30 mg ) in 50 % ethanol .
	manualset3
249526	7	425362	7	NULL	NULL	0	NULL	ethanol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Colitis was induced in rats with intracolonic 2 , 4 , 6-trinitrobenzenesulfonic acid ( TNBS , 30 mg ) in 50 % ethanol .
	manualset3
246078	1	425363	7	NULL	NULL	0	NULL	Collaboration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Collaboration between a hospital-based research team and bedside nurses has produced a successful , funded program of research that has led to dissemination of findings .
	manualset3
246079	2	425363	7	NULL	NULL	0	NULL	hospital-based research team 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Collaboration between a hospital-based research team and bedside nurses has produced a successful , funded program of research that has led to dissemination of findings .
	manualset3
246080	3	425363	7	NULL	NULL	0	NULL	bedside nurses 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Collaboration between a hospital-based research team and bedside nurses has produced a successful , funded program of research that has led to dissemination of findings .
	manualset3
246081	4	425363	7	NULL	NULL	0	NULL	 funded program	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Collaboration between a hospital-based research team and bedside nurses has produced a successful , funded program of research that has led to dissemination of findings .
	manualset3
246082	5	425363	7	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Collaboration between a hospital-based research team and bedside nurses has produced a successful , funded program of research that has led to dissemination of findings .
	manualset3
246083	6	425363	7	NULL	NULL	0	NULL	dissemination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Collaboration between a hospital-based research team and bedside nurses has produced a successful , funded program of research that has led to dissemination of findings .
	manualset3
246084	7	425363	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Collaboration between a hospital-based research team and bedside nurses has produced a successful , funded program of research that has led to dissemination of findings .
	manualset3
246085	1	425364	7	NULL	NULL	0	NULL	Collaborative efforts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Collaborative efforts in future research will lead to a growth in our clinical experience with the utilization of PNS and will help in identifying the best candidates for it .
	manualset3
246086	2	425364	7	NULL	NULL	0	NULL	future research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Collaborative efforts in future research will lead to a growth in our clinical experience with the utilization of PNS and will help in identifying the best candidates for it .
	manualset3
246087	3	425364	7	NULL	NULL	0	NULL	growth	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Collaborative efforts in future research will lead to a growth in our clinical experience with the utilization of PNS and will help in identifying the best candidates for it .
	manualset3
246088	4	425364	7	NULL	NULL	0	NULL	clinical experience	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Collaborative efforts in future research will lead to a growth in our clinical experience with the utilization of PNS and will help in identifying the best candidates for it .
	manualset3
246089	5	425364	7	NULL	NULL	0	NULL	utilization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Collaborative efforts in future research will lead to a growth in our clinical experience with the utilization of PNS and will help in identifying the best candidates for it .
	manualset3
246090	6	425364	7	NULL	NULL	0	NULL	PNS	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Collaborative efforts in future research will lead to a growth in our clinical experience with the utilization of PNS and will help in identifying the best candidates for it .
	manualset3
246091	7	425364	7	NULL	NULL	0	NULL	best candidates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Collaborative efforts in future research will lead to a growth in our clinical experience with the utilization of PNS and will help in identifying the best candidates for it .
	manualset3
246092	1	425365	7	NULL	NULL	0	NULL	Collagens	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Collagens are integral structural proteins in animal tissues and play key functional roles in cellular modulation .
	manualset3
246093	2	425365	7	NULL	NULL	0	NULL	integral structural proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Collagens are integral structural proteins in animal tissues and play key functional roles in cellular modulation .
	manualset3
246094	3	425365	7	NULL	NULL	0	NULL	animal tissues 	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Collagens are integral structural proteins in animal tissues and play key functional roles in cellular modulation .
	manualset3
246095	4	425365	7	NULL	NULL	0	NULL	functional roles	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Collagens are integral structural proteins in animal tissues and play key functional roles in cellular modulation .
	manualset3
246096	5	425365	7	NULL	NULL	0	NULL	cellular modulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Collagens are integral structural proteins in animal tissues and play key functional roles in cellular modulation .
	manualset3
246097	1	425366	7	NULL	NULL	0	NULL	Collection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Collection of peripheral blood CD34 + progenitor cells from healthy dogs and dogs diagnosed with lymphoproliferative diseases using a Baxter-Fenwal CS-3000 Plus blood cell separator .
	manualset3
246098	2	425366	7	NULL	NULL	0	NULL	peripheral blood CD34 + progenitor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Collection of peripheral blood CD34 + progenitor cells from healthy dogs and dogs diagnosed with lymphoproliferative diseases using a Baxter-Fenwal CS-3000 Plus blood cell separator .
	manualset3
246099	3	425366	7	NULL	NULL	0	NULL	healthy dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Collection of peripheral blood CD34 + progenitor cells from healthy dogs and dogs diagnosed with lymphoproliferative diseases using a Baxter-Fenwal CS-3000 Plus blood cell separator .
	manualset3
246100	4	425366	7	NULL	NULL	0	NULL	dogs 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Collection of peripheral blood CD34 + progenitor cells from healthy dogs and dogs diagnosed with lymphoproliferative diseases using a Baxter-Fenwal CS-3000 Plus blood cell separator .
	manualset3
246101	5	425366	7	NULL	NULL	0	NULL	lymphoproliferative diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Collection of peripheral blood CD34 + progenitor cells from healthy dogs and dogs diagnosed with lymphoproliferative diseases using a Baxter-Fenwal CS-3000 Plus blood cell separator .
	manualset3
246102	6	425366	7	NULL	NULL	0	NULL	Baxter-Fenwal CS-3000 Plus blood cell separator	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Collection of peripheral blood CD34 + progenitor cells from healthy dogs and dogs diagnosed with lymphoproliferative diseases using a Baxter-Fenwal CS-3000 Plus blood cell separator .
	manualset3
246103	1	425367	7	NULL	NULL	0	NULL	Intra-articular injections	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intra-articular injections of hyaluronic acid in the treatment of knee osteoarthritis ) .
	manualset3
246104	2	425367	7	NULL	NULL	0	NULL	hyaluronic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intra-articular injections of hyaluronic acid in the treatment of knee osteoarthritis ) .
	manualset3
246105	3	425367	7	NULL	NULL	0	NULL	 treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intra-articular injections of hyaluronic acid in the treatment of knee osteoarthritis ) .
	manualset3
246106	4	425367	7	NULL	NULL	0	NULL	 knee osteoarthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intra-articular injections of hyaluronic acid in the treatment of knee osteoarthritis ) .
	manualset3
246107	1	425368	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , our data suggest that S-nitrosylation of ApoE proteins may play an important role in regulating lipid metabolism and in the pathogenesis of LOAD .
	manualset3
246108	2	425368	7	NULL	NULL	0	NULL	 S-nitrosylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , our data suggest that S-nitrosylation of ApoE proteins may play an important role in regulating lipid metabolism and in the pathogenesis of LOAD .
	manualset3
246109	3	425368	7	NULL	NULL	0	NULL	ApoE proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , our data suggest that S-nitrosylation of ApoE proteins may play an important role in regulating lipid metabolism and in the pathogenesis of LOAD .
	manualset3
246110	4	425368	7	NULL	NULL	0	NULL	 role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , our data suggest that S-nitrosylation of ApoE proteins may play an important role in regulating lipid metabolism and in the pathogenesis of LOAD .
	manualset3
246111	5	425368	7	NULL	NULL	0	NULL	lipid metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , our data suggest that S-nitrosylation of ApoE proteins may play an important role in regulating lipid metabolism and in the pathogenesis of LOAD .
	manualset3
246112	6	425368	7	NULL	NULL	0	NULL	pathogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , our data suggest that S-nitrosylation of ApoE proteins may play an important role in regulating lipid metabolism and in the pathogenesis of LOAD .
	manualset3
246113	7	425368	7	NULL	NULL	0	NULL	LOAD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , our data suggest that S-nitrosylation of ApoE proteins may play an important role in regulating lipid metabolism and in the pathogenesis of LOAD .
	manualset3
246114	1	425369	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , our findings indicate that the degradative fate of the beta ( 2 ) AR in the lysosomal compartments is dependent upon beta-arrestin2-mediated recruitment of Nedd4 to the activated receptor and Nedd4-catalyzed ubiquitination .
	manualset3
246115	2	425369	7	NULL	NULL	0	NULL	degradative fate	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , our findings indicate that the degradative fate of the beta ( 2 ) AR in the lysosomal compartments is dependent upon beta-arrestin2-mediated recruitment of Nedd4 to the activated receptor and Nedd4-catalyzed ubiquitination .
	manualset3
246116	3	425369	7	NULL	NULL	0	NULL	beta ( 2 ) AR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , our findings indicate that the degradative fate of the beta ( 2 ) AR in the lysosomal compartments is dependent upon beta-arrestin2-mediated recruitment of Nedd4 to the activated receptor and Nedd4-catalyzed ubiquitination .
	manualset3
246117	4	425369	7	NULL	NULL	0	NULL	lysosomal compartments	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , our findings indicate that the degradative fate of the beta ( 2 ) AR in the lysosomal compartments is dependent upon beta-arrestin2-mediated recruitment of Nedd4 to the activated receptor and Nedd4-catalyzed ubiquitination .
	manualset3
246118	5	425369	7	NULL	NULL	0	NULL	beta-arrestin2-mediated recruitment	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , our findings indicate that the degradative fate of the beta ( 2 ) AR in the lysosomal compartments is dependent upon beta-arrestin2-mediated recruitment of Nedd4 to the activated receptor and Nedd4-catalyzed ubiquitination .
	manualset3
246119	6	425369	7	NULL	NULL	0	NULL	Nedd4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , our findings indicate that the degradative fate of the beta ( 2 ) AR in the lysosomal compartments is dependent upon beta-arrestin2-mediated recruitment of Nedd4 to the activated receptor and Nedd4-catalyzed ubiquitination .
	manualset3
246120	7	425369	7	NULL	NULL	0	NULL	activated receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , our findings indicate that the degradative fate of the beta ( 2 ) AR in the lysosomal compartments is dependent upon beta-arrestin2-mediated recruitment of Nedd4 to the activated receptor and Nedd4-catalyzed ubiquitination .
	manualset3
246121	8	425369	7	NULL	NULL	0	NULL	Nedd4-catalyzed ubiquitination	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , our findings indicate that the degradative fate of the beta ( 2 ) AR in the lysosomal compartments is dependent upon beta-arrestin2-mediated recruitment of Nedd4 to the activated receptor and Nedd4-catalyzed ubiquitination .
	manualset3
246122	1	425370	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , the results suggest that astrocytes may modulate anti-MOG T cell responses in the CNS .
	manualset3
246123	2	425370	7	NULL	NULL	0	NULL	astrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , the results suggest that astrocytes may modulate anti-MOG T cell responses in the CNS .
	manualset3
246124	3	425370	7	NULL	NULL	0	NULL	anti-MOG T cell responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , the results suggest that astrocytes may modulate anti-MOG T cell responses in the CNS .
	manualset3
246125	4	425370	7	NULL	NULL	0	NULL	CNS	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , the results suggest that astrocytes may modulate anti-MOG T cell responses in the CNS .
	manualset3
246126	1	425371	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these data suggest that C24 : 0 stimulated type II NKT cells may regulate protection from T1D by activating DCs to secrete IL-10 and suppress the activation and expansion of type I iNKT cells and diabetogenic T cells .
	manualset3
246127	2	425371	7	NULL	NULL	0	NULL	 C24 : 0 stimulated type II NKT cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these data suggest that C24 : 0 stimulated type II NKT cells may regulate protection from T1D by activating DCs to secrete IL-10 and suppress the activation and expansion of type I iNKT cells and diabetogenic T cells .
	manualset3
246128	3	425371	7	NULL	NULL	NULL	NULL	 protection	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Collectively , these data suggest that C24 : 0 stimulated type II NKT cells may regulate protection from T1D by activating DCs to secrete IL-10 and suppress the activation and expansion of type I iNKT cells and diabetogenic T cells .
	manualset3
246129	4	425371	7	NULL	NULL	0	NULL	T1D	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these data suggest that C24 : 0 stimulated type II NKT cells may regulate protection from T1D by activating DCs to secrete IL-10 and suppress the activation and expansion of type I iNKT cells and diabetogenic T cells .
	manualset3
246130	5	425371	7	NULL	NULL	0	NULL	DCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these data suggest that C24 : 0 stimulated type II NKT cells may regulate protection from T1D by activating DCs to secrete IL-10 and suppress the activation and expansion of type I iNKT cells and diabetogenic T cells .
	manualset3
246131	6	425371	7	NULL	NULL	0	NULL	IL-10	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these data suggest that C24 : 0 stimulated type II NKT cells may regulate protection from T1D by activating DCs to secrete IL-10 and suppress the activation and expansion of type I iNKT cells and diabetogenic T cells .
	manualset3
246132	7	425371	7	NULL	NULL	0	NULL	activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these data suggest that C24 : 0 stimulated type II NKT cells may regulate protection from T1D by activating DCs to secrete IL-10 and suppress the activation and expansion of type I iNKT cells and diabetogenic T cells .
	manualset3
246133	8	425371	7	NULL	NULL	0	NULL	expansion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these data suggest that C24 : 0 stimulated type II NKT cells may regulate protection from T1D by activating DCs to secrete IL-10 and suppress the activation and expansion of type I iNKT cells and diabetogenic T cells .
	manualset3
246134	9	425371	7	NULL	NULL	0	NULL	type I iNKT cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these data suggest that C24 : 0 stimulated type II NKT cells may regulate protection from T1D by activating DCs to secrete IL-10 and suppress the activation and expansion of type I iNKT cells and diabetogenic T cells .
	manualset3
246135	10	425371	7	NULL	NULL	0	NULL	 diabetogenic T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these data suggest that C24 : 0 stimulated type II NKT cells may regulate protection from T1D by activating DCs to secrete IL-10 and suppress the activation and expansion of type I iNKT cells and diabetogenic T cells .
	manualset3
246142	1	425373	7	NULL	NULL	0	NULL	 findings 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these findings suggest that SUMO-1 modification of MDA5 possibly via PIAS2 may play a role in the MDA5-mediated IFN response to viral infections .
	manualset3
246143	2	425373	7	NULL	NULL	0	NULL	SUMO-1 modification	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these findings suggest that SUMO-1 modification of MDA5 possibly via PIAS2 may play a role in the MDA5-mediated IFN response to viral infections .
	manualset3
246144	3	425373	7	NULL	NULL	0	NULL	MDA5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these findings suggest that SUMO-1 modification of MDA5 possibly via PIAS2 may play a role in the MDA5-mediated IFN response to viral infections .
	manualset3
246145	4	425373	7	NULL	NULL	0	NULL	 PIAS2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these findings suggest that SUMO-1 modification of MDA5 possibly via PIAS2 may play a role in the MDA5-mediated IFN response to viral infections .
	manualset3
246146	5	425373	7	NULL	NULL	0	NULL	role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these findings suggest that SUMO-1 modification of MDA5 possibly via PIAS2 may play a role in the MDA5-mediated IFN response to viral infections .
	manualset3
246147	6	425373	7	NULL	NULL	0	NULL	MDA5-mediated IFN response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these findings suggest that SUMO-1 modification of MDA5 possibly via PIAS2 may play a role in the MDA5-mediated IFN response to viral infections .
	manualset3
246148	7	425373	7	NULL	NULL	0	NULL	viral infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these findings suggest that SUMO-1 modification of MDA5 possibly via PIAS2 may play a role in the MDA5-mediated IFN response to viral infections .
	manualset3
246149	1	425374	7	NULL	NULL	0	NULL	 findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these findings support a paradigm in which the stimulation of DC , T cells , and the tumor vasculature by an OX40 agonist dynamically orchestrates the activation , expansion , and recruitment of therapeutic T cells into established tumors .
	manualset3
246150	2	425374	7	NULL	NULL	0	NULL	paradigm	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these findings support a paradigm in which the stimulation of DC , T cells , and the tumor vasculature by an OX40 agonist dynamically orchestrates the activation , expansion , and recruitment of therapeutic T cells into established tumors .
	manualset3
246151	3	425374	7	NULL	NULL	0	NULL	stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these findings support a paradigm in which the stimulation of DC , T cells , and the tumor vasculature by an OX40 agonist dynamically orchestrates the activation , expansion , and recruitment of therapeutic T cells into established tumors .
	manualset3
246152	4	425374	7	NULL	NULL	0	NULL	DC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these findings support a paradigm in which the stimulation of DC , T cells , and the tumor vasculature by an OX40 agonist dynamically orchestrates the activation , expansion , and recruitment of therapeutic T cells into established tumors .
	manualset3
246153	5	425374	7	NULL	NULL	0	NULL	T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these findings support a paradigm in which the stimulation of DC , T cells , and the tumor vasculature by an OX40 agonist dynamically orchestrates the activation , expansion , and recruitment of therapeutic T cells into established tumors .
	manualset3
246154	6	425374	7	NULL	NULL	0	NULL	 tumor vasculature	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these findings support a paradigm in which the stimulation of DC , T cells , and the tumor vasculature by an OX40 agonist dynamically orchestrates the activation , expansion , and recruitment of therapeutic T cells into established tumors .
	manualset3
246155	7	425374	7	NULL	NULL	0	NULL	OX40 agonist	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these findings support a paradigm in which the stimulation of DC , T cells , and the tumor vasculature by an OX40 agonist dynamically orchestrates the activation , expansion , and recruitment of therapeutic T cells into established tumors .
	manualset3
246156	8	425374	7	NULL	NULL	0	NULL	activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these findings support a paradigm in which the stimulation of DC , T cells , and the tumor vasculature by an OX40 agonist dynamically orchestrates the activation , expansion , and recruitment of therapeutic T cells into established tumors .
	manualset3
246157	9	425374	7	NULL	NULL	0	NULL	expansion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these findings support a paradigm in which the stimulation of DC , T cells , and the tumor vasculature by an OX40 agonist dynamically orchestrates the activation , expansion , and recruitment of therapeutic T cells into established tumors .
	manualset3
246158	10	425374	7	NULL	NULL	0	NULL	recruitment	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these findings support a paradigm in which the stimulation of DC , T cells , and the tumor vasculature by an OX40 agonist dynamically orchestrates the activation , expansion , and recruitment of therapeutic T cells into established tumors .
	manualset3
246159	11	425374	7	NULL	NULL	0	NULL	therapeutic T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these findings support a paradigm in which the stimulation of DC , T cells , and the tumor vasculature by an OX40 agonist dynamically orchestrates the activation , expansion , and recruitment of therapeutic T cells into established tumors .
	manualset3
246160	12	425374	7	NULL	NULL	0	NULL	 tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these findings support a paradigm in which the stimulation of DC , T cells , and the tumor vasculature by an OX40 agonist dynamically orchestrates the activation , expansion , and recruitment of therapeutic T cells into established tumors .
	manualset3
246161	1	425375	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these results indicate that mechanistically diverse tumor promoter stimuli elevate TGF alpha mRNA and protein in SENCAR mouse epidermis .
	manualset3
246162	2	425375	7	NULL	NULL	0	NULL	tumor promoter stimuli	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these results indicate that mechanistically diverse tumor promoter stimuli elevate TGF alpha mRNA and protein in SENCAR mouse epidermis .
	manualset3
246163	3	425375	7	NULL	NULL	0	NULL	TGF alpha mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these results indicate that mechanistically diverse tumor promoter stimuli elevate TGF alpha mRNA and protein in SENCAR mouse epidermis .
	manualset3
246164	4	425375	7	NULL	NULL	0	NULL	protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these results indicate that mechanistically diverse tumor promoter stimuli elevate TGF alpha mRNA and protein in SENCAR mouse epidermis .
	manualset3
246165	5	425375	7	NULL	NULL	0	NULL	SENCAR mouse epidermis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these results indicate that mechanistically diverse tumor promoter stimuli elevate TGF alpha mRNA and protein in SENCAR mouse epidermis .
	manualset3
246227	1	425376	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these results suggest that the GABA-modulatory effects of physiological levels of the neurosteroid will not be uniformly experienced throughout the central nervous system , or even within the same brain region such as the hippocampus , but will be neurone-specific and will be dependent on the phosphorylation status of the GABA ( A ) receptor , or associated proteins .
	manualset3
246228	2	425376	7	NULL	NULL	0	NULL	GABA-modulatory effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these results suggest that the GABA-modulatory effects of physiological levels of the neurosteroid will not be uniformly experienced throughout the central nervous system , or even within the same brain region such as the hippocampus , but will be neurone-specific and will be dependent on the phosphorylation status of the GABA ( A ) receptor , or associated proteins .
	manualset3
246229	3	425376	7	NULL	NULL	0	NULL	physiological levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these results suggest that the GABA-modulatory effects of physiological levels of the neurosteroid will not be uniformly experienced throughout the central nervous system , or even within the same brain region such as the hippocampus , but will be neurone-specific and will be dependent on the phosphorylation status of the GABA ( A ) receptor , or associated proteins .
	manualset3
246230	4	425376	7	NULL	NULL	0	NULL	 neurosteroid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these results suggest that the GABA-modulatory effects of physiological levels of the neurosteroid will not be uniformly experienced throughout the central nervous system , or even within the same brain region such as the hippocampus , but will be neurone-specific and will be dependent on the phosphorylation status of the GABA ( A ) receptor , or associated proteins .
	manualset3
246231	5	425376	7	NULL	NULL	0	NULL	central nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these results suggest that the GABA-modulatory effects of physiological levels of the neurosteroid will not be uniformly experienced throughout the central nervous system , or even within the same brain region such as the hippocampus , but will be neurone-specific and will be dependent on the phosphorylation status of the GABA ( A ) receptor , or associated proteins .
	manualset3
246232	6	425376	7	NULL	NULL	0	NULL	brain region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these results suggest that the GABA-modulatory effects of physiological levels of the neurosteroid will not be uniformly experienced throughout the central nervous system , or even within the same brain region such as the hippocampus , but will be neurone-specific and will be dependent on the phosphorylation status of the GABA ( A ) receptor , or associated proteins .
	manualset3
246233	7	425376	7	NULL	NULL	0	NULL	hippocampus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these results suggest that the GABA-modulatory effects of physiological levels of the neurosteroid will not be uniformly experienced throughout the central nervous system , or even within the same brain region such as the hippocampus , but will be neurone-specific and will be dependent on the phosphorylation status of the GABA ( A ) receptor , or associated proteins .
	manualset3
246234	8	425376	7	NULL	NULL	0	NULL	phosphorylation status 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these results suggest that the GABA-modulatory effects of physiological levels of the neurosteroid will not be uniformly experienced throughout the central nervous system , or even within the same brain region such as the hippocampus , but will be neurone-specific and will be dependent on the phosphorylation status of the GABA ( A ) receptor , or associated proteins .
	manualset3
246235	9	425376	7	NULL	NULL	0	NULL	GABA ( A ) receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively , these results suggest that the GABA-modulatory effects of physiological levels of the neurosteroid will not be uniformly experienced throughout the central nervous system , or even within the same brain region such as the hippocampus , but will be neurone-specific and will be dependent on the phosphorylation status of the GABA ( A ) receptor , or associated proteins .
	manualset3
246236	10	425376	7	NULL	NULL	NULL	NULL	associated proteins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Collectively , these results suggest that the GABA-modulatory effects of physiological levels of the neurosteroid will not be uniformly experienced throughout the central nervous system , or even within the same brain region such as the hippocampus , but will be neurone-specific and will be dependent on the phosphorylation status of the GABA ( A ) receptor , or associated proteins .
	manualset3
246237	1	425377	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively these findings document that the MRL-lpr/lpr mice spontaneously develop autoimmune thyroiditis and can be used as a model for the study of thyroid-specific autoimmunity .
	manualset3
246238	2	425377	7	NULL	NULL	0	NULL	MRL-lpr/lpr mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively these findings document that the MRL-lpr/lpr mice spontaneously develop autoimmune thyroiditis and can be used as a model for the study of thyroid-specific autoimmunity .
	manualset3
246239	3	425377	7	NULL	NULL	0	NULL	autoimmune thyroiditis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively these findings document that the MRL-lpr/lpr mice spontaneously develop autoimmune thyroiditis and can be used as a model for the study of thyroid-specific autoimmunity .
	manualset3
246240	4	425377	7	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively these findings document that the MRL-lpr/lpr mice spontaneously develop autoimmune thyroiditis and can be used as a model for the study of thyroid-specific autoimmunity .
	manualset3
246241	5	425377	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively these findings document that the MRL-lpr/lpr mice spontaneously develop autoimmune thyroiditis and can be used as a model for the study of thyroid-specific autoimmunity .
	manualset3
246242	6	425377	7	NULL	NULL	0	NULL	thyroid-specific autoimmunity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Collectively these findings document that the MRL-lpr/lpr mice spontaneously develop autoimmune thyroiditis and can be used as a model for the study of thyroid-specific autoimmunity .
	manualset3
246243	1	425378	7	NULL	NULL	0	NULL	College-aged individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	College-aged individuals are at risk for bicycle-related head injuries , but the risk of such injuries can be reduced by their use of bicycle helmets .
	manualset3
246244	2	425378	7	NULL	NULL	0	NULL	 risk 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	College-aged individuals are at risk for bicycle-related head injuries , but the risk of such injuries can be reduced by their use of bicycle helmets .
	manualset3
246245	3	425378	7	NULL	NULL	0	NULL	 bicycle-related head injuries	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	College-aged individuals are at risk for bicycle-related head injuries , but the risk of such injuries can be reduced by their use of bicycle helmets .
	manualset3
246246	4	425378	7	NULL	NULL	0	NULL	 risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	College-aged individuals are at risk for bicycle-related head injuries , but the risk of such injuries can be reduced by their use of bicycle helmets .
	manualset3
246247	5	425378	7	NULL	NULL	0	NULL	 injuries	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	College-aged individuals are at risk for bicycle-related head injuries , but the risk of such injuries can be reduced by their use of bicycle helmets .
	manualset3
246248	6	425378	7	NULL	NULL	0	NULL	 use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	College-aged individuals are at risk for bicycle-related head injuries , but the risk of such injuries can be reduced by their use of bicycle helmets .
	manualset3
246249	7	425378	7	NULL	NULL	NULL	NULL	bicycle helmets	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	College-aged individuals are at risk for bicycle-related head injuries , but the risk of such injuries can be reduced by their use of bicycle helmets .
	manualset3
246260	1	425379	7	NULL	NULL	0	NULL	Colonic mucosal mRNA expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonic mucosal mRNA expression of critical Th17 cell cytokines and chemokine receptors ( IL-17F , IL-21 , and CCR6 ) were lower , whereas expression of the Th17 cell suppressive cytokine , IL-27 , was greater in Fat-1 mice compared to WT mice during chronic colitis ( P & lt ; 0.05 ) .
	manualset3
246261	2	425379	7	NULL	NULL	0	NULL	critical Th17 cell cytokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonic mucosal mRNA expression of critical Th17 cell cytokines and chemokine receptors ( IL-17F , IL-21 , and CCR6 ) were lower , whereas expression of the Th17 cell suppressive cytokine , IL-27 , was greater in Fat-1 mice compared to WT mice during chronic colitis ( P & lt ; 0.05 ) .
	manualset3
246262	3	425379	7	NULL	NULL	0	NULL	chemokine receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonic mucosal mRNA expression of critical Th17 cell cytokines and chemokine receptors ( IL-17F , IL-21 , and CCR6 ) were lower , whereas expression of the Th17 cell suppressive cytokine , IL-27 , was greater in Fat-1 mice compared to WT mice during chronic colitis ( P & lt ; 0.05 ) .
	manualset3
246263	4	425379	7	NULL	NULL	0	NULL	IL-17F	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonic mucosal mRNA expression of critical Th17 cell cytokines and chemokine receptors ( IL-17F , IL-21 , and CCR6 ) were lower , whereas expression of the Th17 cell suppressive cytokine , IL-27 , was greater in Fat-1 mice compared to WT mice during chronic colitis ( P & lt ; 0.05 ) .
	manualset3
246264	5	425379	7	NULL	NULL	0	NULL	IL-21	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonic mucosal mRNA expression of critical Th17 cell cytokines and chemokine receptors ( IL-17F , IL-21 , and CCR6 ) were lower , whereas expression of the Th17 cell suppressive cytokine , IL-27 , was greater in Fat-1 mice compared to WT mice during chronic colitis ( P & lt ; 0.05 ) .
	manualset3
246265	6	425379	7	NULL	NULL	0	NULL	CCR6	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonic mucosal mRNA expression of critical Th17 cell cytokines and chemokine receptors ( IL-17F , IL-21 , and CCR6 ) were lower , whereas expression of the Th17 cell suppressive cytokine , IL-27 , was greater in Fat-1 mice compared to WT mice during chronic colitis ( P & lt ; 0.05 ) .
	manualset3
246266	7	425379	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonic mucosal mRNA expression of critical Th17 cell cytokines and chemokine receptors ( IL-17F , IL-21 , and CCR6 ) were lower , whereas expression of the Th17 cell suppressive cytokine , IL-27 , was greater in Fat-1 mice compared to WT mice during chronic colitis ( P & lt ; 0.05 ) .
	manualset3
246267	8	425379	7	NULL	NULL	0	NULL	Th17 cell suppressive cytokine	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonic mucosal mRNA expression of critical Th17 cell cytokines and chemokine receptors ( IL-17F , IL-21 , and CCR6 ) were lower , whereas expression of the Th17 cell suppressive cytokine , IL-27 , was greater in Fat-1 mice compared to WT mice during chronic colitis ( P & lt ; 0.05 ) .
	manualset3
246268	9	425379	7	NULL	NULL	0	NULL	IL-27	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonic mucosal mRNA expression of critical Th17 cell cytokines and chemokine receptors ( IL-17F , IL-21 , and CCR6 ) were lower , whereas expression of the Th17 cell suppressive cytokine , IL-27 , was greater in Fat-1 mice compared to WT mice during chronic colitis ( P & lt ; 0.05 ) .
	manualset3
246269	10	425379	7	NULL	NULL	0	NULL	Fat-1 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonic mucosal mRNA expression of critical Th17 cell cytokines and chemokine receptors ( IL-17F , IL-21 , and CCR6 ) were lower , whereas expression of the Th17 cell suppressive cytokine , IL-27 , was greater in Fat-1 mice compared to WT mice during chronic colitis ( P & lt ; 0.05 ) .
	manualset3
246270	11	425379	7	NULL	NULL	0	NULL	WT mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonic mucosal mRNA expression of critical Th17 cell cytokines and chemokine receptors ( IL-17F , IL-21 , and CCR6 ) were lower , whereas expression of the Th17 cell suppressive cytokine , IL-27 , was greater in Fat-1 mice compared to WT mice during chronic colitis ( P & lt ; 0.05 ) .
	manualset3
246271	12	425379	7	NULL	NULL	0	NULL	chronic colitis 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonic mucosal mRNA expression of critical Th17 cell cytokines and chemokine receptors ( IL-17F , IL-21 , and CCR6 ) were lower , whereas expression of the Th17 cell suppressive cytokine , IL-27 , was greater in Fat-1 mice compared to WT mice during chronic colitis ( P & lt ; 0.05 ) .
	manualset3
246272	13	425379	7	NULL	NULL	0	NULL	P & lt ; 0.05	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonic mucosal mRNA expression of critical Th17 cell cytokines and chemokine receptors ( IL-17F , IL-21 , and CCR6 ) were lower , whereas expression of the Th17 cell suppressive cytokine , IL-27 , was greater in Fat-1 mice compared to WT mice during chronic colitis ( P & lt ; 0.05 ) .
	manualset3
246273	1	425380	7	NULL	NULL	0	NULL	Colonies 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonies of Thiobacillus thioparus and T. thiooxidans grown on thiosulfate medium can be identified by replica plating on thallous sulfide paper .
	manualset3
246274	2	425380	7	NULL	NULL	0	NULL	Thiobacillus thioparus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonies of Thiobacillus thioparus and T. thiooxidans grown on thiosulfate medium can be identified by replica plating on thallous sulfide paper .
	manualset3
246275	3	425380	7	NULL	NULL	0	NULL	T. thiooxidans 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonies of Thiobacillus thioparus and T. thiooxidans grown on thiosulfate medium can be identified by replica plating on thallous sulfide paper .
	manualset3
246276	4	425380	7	NULL	NULL	0	NULL	thiosulfate medium 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonies of Thiobacillus thioparus and T. thiooxidans grown on thiosulfate medium can be identified by replica plating on thallous sulfide paper .
	manualset3
246277	5	425380	7	NULL	NULL	0	NULL	replica plating 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonies of Thiobacillus thioparus and T. thiooxidans grown on thiosulfate medium can be identified by replica plating on thallous sulfide paper .
	manualset3
246278	6	425380	7	NULL	NULL	0	NULL	thallous sulfide paper	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonies of Thiobacillus thioparus and T. thiooxidans grown on thiosulfate medium can be identified by replica plating on thallous sulfide paper .
	manualset3
246279	1	425381	7	NULL	NULL	0	NULL	Colonization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonization of plants by nonpathogenic Pseudomonas fluorescens strains can confer enhanced defense capacity against a broad spectrum of pathogens .
	manualset3
246280	2	425381	7	NULL	NULL	0	NULL	plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonization of plants by nonpathogenic Pseudomonas fluorescens strains can confer enhanced defense capacity against a broad spectrum of pathogens .
	manualset3
246332	3	425381	7	NULL	NULL	0	NULL	nonpathogenic Pseudomonas fluorescens strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonization of plants by nonpathogenic Pseudomonas fluorescens strains can confer enhanced defense capacity against a broad spectrum of pathogens .
	manualset3
246333	4	425381	7	NULL	NULL	0	NULL	 defense capacity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonization of plants by nonpathogenic Pseudomonas fluorescens strains can confer enhanced defense capacity against a broad spectrum of pathogens .
	manualset3
246334	5	425381	7	NULL	NULL	0	NULL	broad spectrum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonization of plants by nonpathogenic Pseudomonas fluorescens strains can confer enhanced defense capacity against a broad spectrum of pathogens .
	manualset3
246335	6	425381	7	NULL	NULL	0	NULL	 pathogens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonization of plants by nonpathogenic Pseudomonas fluorescens strains can confer enhanced defense capacity against a broad spectrum of pathogens .
	manualset3
246336	1	425382	7	NULL	NULL	0	NULL	Colonoscopic removal	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonoscopic removal of polyps reduces cancer risk .
	manualset3
246337	2	425382	7	NULL	NULL	0	NULL	 polyps	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonoscopic removal of polyps reduces cancer risk .
	manualset3
246338	3	425382	7	NULL	NULL	0	NULL	 cancer risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Colonoscopic removal of polyps reduces cancer risk .
	manualset3
246339	1	425383	7	NULL	NULL	0	NULL	Color change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Color change indicating the presence of carbon dioxide without subsequent color change back to purple with insufflation with 100 % oxygen should arouse suspicion of improper placement of the endotracheal tube .
	manualset3
246340	2	425383	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Color change indicating the presence of carbon dioxide without subsequent color change back to purple with insufflation with 100 % oxygen should arouse suspicion of improper placement of the endotracheal tube .
	manualset3
246341	3	425383	7	NULL	NULL	0	NULL	carbon dioxide 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Color change indicating the presence of carbon dioxide without subsequent color change back to purple with insufflation with 100 % oxygen should arouse suspicion of improper placement of the endotracheal tube .
	manualset3
246342	4	425383	7	NULL	NULL	0	NULL	Color change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Color change indicating the presence of carbon dioxide without subsequent color change back to purple with insufflation with 100 % oxygen should arouse suspicion of improper placement of the endotracheal tube .
	manualset3
246343	5	425383	7	NULL	NULL	0	NULL	purple	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Color change indicating the presence of carbon dioxide without subsequent color change back to purple with insufflation with 100 % oxygen should arouse suspicion of improper placement of the endotracheal tube .
	manualset3
246344	6	425383	7	NULL	NULL	0	NULL	 insufflation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Color change indicating the presence of carbon dioxide without subsequent color change back to purple with insufflation with 100 % oxygen should arouse suspicion of improper placement of the endotracheal tube .
	manualset3
246345	7	425383	7	NULL	NULL	0	NULL	100 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Color change indicating the presence of carbon dioxide without subsequent color change back to purple with insufflation with 100 % oxygen should arouse suspicion of improper placement of the endotracheal tube .
	manualset3
246346	8	425383	7	NULL	NULL	0	NULL	oxygen	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Color change indicating the presence of carbon dioxide without subsequent color change back to purple with insufflation with 100 % oxygen should arouse suspicion of improper placement of the endotracheal tube .
	manualset3
246347	9	425383	7	NULL	NULL	0	NULL	suspicion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Color change indicating the presence of carbon dioxide without subsequent color change back to purple with insufflation with 100 % oxygen should arouse suspicion of improper placement of the endotracheal tube .
	manualset3
246348	10	425383	7	NULL	NULL	0	NULL	improper placement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Color change indicating the presence of carbon dioxide without subsequent color change back to purple with insufflation with 100 % oxygen should arouse suspicion of improper placement of the endotracheal tube .
	manualset3
246349	11	425383	7	NULL	NULL	0	NULL	endotracheal tube	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Color change indicating the presence of carbon dioxide without subsequent color change back to purple with insufflation with 100 % oxygen should arouse suspicion of improper placement of the endotracheal tube .
	manualset3
246350	1	425384	7	NULL	NULL	0	NULL	 Intravenous cholangiocholecystography 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intravenous cholangiocholecystography : opacification of the intrahepatic and extrahepatic bile ducts by a new substance ) .
	manualset3
246351	2	425384	7	NULL	NULL	0	NULL	 opacification 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intravenous cholangiocholecystography : opacification of the intrahepatic and extrahepatic bile ducts by a new substance ) .
	manualset3
246352	3	425384	7	NULL	NULL	0	NULL	intrahepatic bile ducts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intravenous cholangiocholecystography : opacification of the intrahepatic and extrahepatic bile ducts by a new substance ) .
	manualset3
246353	4	425384	7	NULL	NULL	0	NULL	extrahepatic bile ducts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intravenous cholangiocholecystography : opacification of the intrahepatic and extrahepatic bile ducts by a new substance ) .
	manualset3
246354	5	425384	7	NULL	NULL	0	NULL	new substance	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Intravenous cholangiocholecystography : opacification of the intrahepatic and extrahepatic bile ducts by a new substance ) .
	manualset3
246355	1	425385	7	NULL	NULL	0	NULL	Color	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Color was measured with two instruments on pork chops of varied ultimate pH ( 5.1-6 .1 ) in a vacuum package and again after blooming .
	manualset3
246356	2	425385	7	NULL	NULL	0	NULL	two instruments	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Color was measured with two instruments on pork chops of varied ultimate pH ( 5.1-6 .1 ) in a vacuum package and again after blooming .
	manualset3
246357	3	425385	7	NULL	NULL	0	NULL	pork chops	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Color was measured with two instruments on pork chops of varied ultimate pH ( 5.1-6 .1 ) in a vacuum package and again after blooming .
	manualset3
246358	4	425385	7	NULL	NULL	0	NULL	pH	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Color was measured with two instruments on pork chops of varied ultimate pH ( 5.1-6 .1 ) in a vacuum package and again after blooming .
	manualset3
246359	5	425385	7	NULL	NULL	0	NULL	5.1-6 .1	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Color was measured with two instruments on pork chops of varied ultimate pH ( 5.1-6 .1 ) in a vacuum package and again after blooming .
	manualset3
246360	6	425385	7	NULL	NULL	0	NULL	vacuum package	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Color was measured with two instruments on pork chops of varied ultimate pH ( 5.1-6 .1 ) in a vacuum package and again after blooming .
	manualset3
246361	7	425385	7	NULL	NULL	0	NULL	blooming	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Color was measured with two instruments on pork chops of varied ultimate pH ( 5.1-6 .1 ) in a vacuum package and again after blooming .
	manualset3
246362	1	425386	7	NULL	NULL	0	NULL	Color Tuning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Color Tuning in rhodopsins : the origin of the spectral shift between the chloride-bound and anion-free forms of halorhodopsin .
	manualset3
246363	2	425386	7	NULL	NULL	0	NULL	rhodopsins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Color Tuning in rhodopsins : the origin of the spectral shift between the chloride-bound and anion-free forms of halorhodopsin .
	manualset3
246364	3	425386	7	NULL	NULL	0	NULL	origin	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Color Tuning in rhodopsins : the origin of the spectral shift between the chloride-bound and anion-free forms of halorhodopsin .
	manualset3
246365	4	425386	7	NULL	NULL	0	NULL	spectral shift 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Color Tuning in rhodopsins : the origin of the spectral shift between the chloride-bound and anion-free forms of halorhodopsin .
	manualset3
246366	5	425386	7	NULL	NULL	0	NULL	chloride-bound halorhodopsin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Color Tuning in rhodopsins : the origin of the spectral shift between the chloride-bound and anion-free forms of halorhodopsin .
	manualset3
246367	6	425386	7	NULL	NULL	0	NULL	anion-free forms of halorhodopsin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Color Tuning in rhodopsins : the origin of the spectral shift between the chloride-bound and anion-free forms of halorhodopsin .
	manualset3
246368	1	425387	7	NULL	NULL	0	NULL	Colorectal cancer ( CRC )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Colorectal cancer ( CRC ) develops through several histologically well-defined stages , reflecting the sequential acquisition of genetic alterations .
	manualset3
246369	2	425387	7	NULL	NULL	0	NULL	well-defined stages	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Colorectal cancer ( CRC ) develops through several histologically well-defined stages , reflecting the sequential acquisition of genetic alterations .
	manualset3
246370	3	425387	7	NULL	NULL	0	NULL	sequential acquisition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Colorectal cancer ( CRC ) develops through several histologically well-defined stages , reflecting the sequential acquisition of genetic alterations .
	manualset3
246371	4	425387	7	NULL	NULL	0	NULL	genetic alterations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Colorectal cancer ( CRC ) develops through several histologically well-defined stages , reflecting the sequential acquisition of genetic alterations .
	manualset3
246372	1	425388	7	NULL	NULL	0	NULL	Colorectal cancer screening	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Colorectal cancer screening : making sense of the different guidelines .
	manualset3
246373	2	425388	7	NULL	NULL	0	NULL	guidelines	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Colorectal cancer screening : making sense of the different guidelines .
	manualset3
246374	1	425389	7	NULL	NULL	0	NULL	Colorimetric microassay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Colorimetric microassay was used to determine lipase activity .
	manualset3
246375	2	425389	7	NULL	NULL	0	NULL	lipase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Colorimetric microassay was used to determine lipase activity .
	manualset3
246376	1	425390	7	NULL	NULL	0	NULL	Colpermin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Colpermin is effective and safe as a therapeutic agent in patients with IBS suffering from abdominal pain or discomfort .
	manualset3
246377	2	425390	7	NULL	NULL	0	NULL	therapeutic agent	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Colpermin is effective and safe as a therapeutic agent in patients with IBS suffering from abdominal pain or discomfort .
	manualset3
246378	3	425390	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Colpermin is effective and safe as a therapeutic agent in patients with IBS suffering from abdominal pain or discomfort .
	manualset3
246379	4	425390	7	NULL	NULL	0	NULL	IBS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Colpermin is effective and safe as a therapeutic agent in patients with IBS suffering from abdominal pain or discomfort .
	manualset3
246380	5	425390	7	NULL	NULL	0	NULL	abdominal pain 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Colpermin is effective and safe as a therapeutic agent in patients with IBS suffering from abdominal pain or discomfort .
	manualset3
246381	6	425390	7	NULL	NULL	0	NULL	discomfort	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Colpermin is effective and safe as a therapeutic agent in patients with IBS suffering from abdominal pain or discomfort .
	manualset3
246429	1	425391	7	NULL	NULL	0	NULL	Column fractions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Column fractions were assayed for the presence of IgM and IgG by immunoblot probing using anti-human IgM and anti-human IgG alkaline phosphatase conjugates .
	manualset3
246430	2	425391	7	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Column fractions were assayed for the presence of IgM and IgG by immunoblot probing using anti-human IgM and anti-human IgG alkaline phosphatase conjugates .
	manualset3
246431	3	425391	7	NULL	NULL	0	NULL	IgM	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Column fractions were assayed for the presence of IgM and IgG by immunoblot probing using anti-human IgM and anti-human IgG alkaline phosphatase conjugates .
	manualset3
246432	4	425391	7	NULL	NULL	0	NULL	IgG 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Column fractions were assayed for the presence of IgM and IgG by immunoblot probing using anti-human IgM and anti-human IgG alkaline phosphatase conjugates .
	manualset3
246433	5	425391	7	NULL	NULL	0	NULL	immunoblot probing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Column fractions were assayed for the presence of IgM and IgG by immunoblot probing using anti-human IgM and anti-human IgG alkaline phosphatase conjugates .
	manualset3
246434	6	425391	7	NULL	NULL	0	NULL	anti-human IgM alkaline phosphatase conjugates	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Column fractions were assayed for the presence of IgM and IgG by immunoblot probing using anti-human IgM and anti-human IgG alkaline phosphatase conjugates .
	manualset3
246435	7	425391	7	NULL	NULL	0	NULL	anti-human IgG alkaline phosphatase conjugates	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Column fractions were assayed for the presence of IgM and IgG by immunoblot probing using anti-human IgM and anti-human IgG alkaline phosphatase conjugates .
	manualset3
246438	1	425392	7	NULL	NULL	0	NULL	Column liquid chromatography-ultraviolet evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Column liquid chromatography-ultraviolet and column liquid chromatography/mass spectrometry evaluation of stress degradation behavior of escitalopram oxalate .
	manualset3
246440	2	425392	7	NULL	NULL	0	NULL	column liquid chromatography/mass spectrometry evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Column liquid chromatography-ultraviolet and column liquid chromatography/mass spectrometry evaluation of stress degradation behavior of escitalopram oxalate .
	manualset3
246441	3	425392	7	NULL	NULL	0	NULL	stress degradation behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Column liquid chromatography-ultraviolet and column liquid chromatography/mass spectrometry evaluation of stress degradation behavior of escitalopram oxalate .
	manualset3
246442	4	425392	7	NULL	NULL	0	NULL	escitalopram oxalate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Column liquid chromatography-ultraviolet and column liquid chromatography/mass spectrometry evaluation of stress degradation behavior of escitalopram oxalate .
	manualset3
246443	1	425393	7	NULL	NULL	0	NULL	Combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination of both maneuvers : perfusion with a K + - free and Ba2 + - containing solution almost abolished Isc from a control of 237 to 56 microA X cm-2 .
	manualset3
246447	2	425393	7	NULL	NULL	0	NULL	maneuvers	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination of both maneuvers : perfusion with a K + - free and Ba2 + - containing solution almost abolished Isc from a control of 237 to 56 microA X cm-2 .
	manualset3
246453	3	425393	7	NULL	NULL	0	NULL	 perfusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination of both maneuvers : perfusion with a K + - free and Ba2 + - containing solution almost abolished Isc from a control of 237 to 56 microA X cm-2 .
	manualset3
246454	4	425393	7	NULL	NULL	0	NULL	K + - free containing solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination of both maneuvers : perfusion with a K + - free and Ba2 + - containing solution almost abolished Isc from a control of 237 to 56 microA X cm-2 .
	manualset3
246455	5	425393	7	NULL	NULL	0	NULL	Ba2 + - containing solution	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination of both maneuvers : perfusion with a K + - free and Ba2 + - containing solution almost abolished Isc from a control of 237 to 56 microA X cm-2 .
	manualset3
246456	6	425393	7	NULL	NULL	0	NULL	Isc	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination of both maneuvers : perfusion with a K + - free and Ba2 + - containing solution almost abolished Isc from a control of 237 to 56 microA X cm-2 .
	manualset3
246467	7	425393	7	NULL	NULL	0	NULL	control	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination of both maneuvers : perfusion with a K + - free and Ba2 + - containing solution almost abolished Isc from a control of 237 to 56 microA X cm-2 .
	manualset3
246468	8	425393	7	NULL	NULL	0	NULL	 237	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination of both maneuvers : perfusion with a K + - free and Ba2 + - containing solution almost abolished Isc from a control of 237 to 56 microA X cm-2 .
	manualset3
246469	9	425393	7	NULL	NULL	0	NULL	56 microA X cm-2	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination of both maneuvers : perfusion with a K + - free and Ba2 + - containing solution almost abolished Isc from a control of 237 to 56 microA X cm-2 .
	manualset3
246541	1	425394	7	NULL	NULL	0	NULL	Introduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Introduction : update in cardiology ) .
	manualset3
246542	2	425394	7	NULL	NULL	0	NULL	update	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Introduction : update in cardiology ) .
	manualset3
246543	3	425394	7	NULL	NULL	0	NULL	cardiology 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Introduction : update in cardiology ) .
	manualset3
246544	1	425395	7	NULL	NULL	0	NULL	Combination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination of detoxifying liver support systems with liver cell bioreactors may have additional benefits for the treatment of liver failure due to the replacement of known and unknown metabolic activities of the liver .
	manualset3
246545	2	425395	7	NULL	NULL	0	NULL	detoxifying liver support systems	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination of detoxifying liver support systems with liver cell bioreactors may have additional benefits for the treatment of liver failure due to the replacement of known and unknown metabolic activities of the liver .
	manualset3
246546	3	425395	7	NULL	NULL	0	NULL	liver cell bioreactors	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination of detoxifying liver support systems with liver cell bioreactors may have additional benefits for the treatment of liver failure due to the replacement of known and unknown metabolic activities of the liver .
	manualset3
246547	4	425395	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination of detoxifying liver support systems with liver cell bioreactors may have additional benefits for the treatment of liver failure due to the replacement of known and unknown metabolic activities of the liver .
	manualset3
246548	5	425395	7	NULL	NULL	0	NULL	liver failure 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination of detoxifying liver support systems with liver cell bioreactors may have additional benefits for the treatment of liver failure due to the replacement of known and unknown metabolic activities of the liver .
	manualset3
246549	6	425395	7	NULL	NULL	0	NULL	replacement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination of detoxifying liver support systems with liver cell bioreactors may have additional benefits for the treatment of liver failure due to the replacement of known and unknown metabolic activities of the liver .
	manualset3
246550	7	425395	7	NULL	NULL	0	NULL	metabolic activities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination of detoxifying liver support systems with liver cell bioreactors may have additional benefits for the treatment of liver failure due to the replacement of known and unknown metabolic activities of the liver .
	manualset3
246551	8	425395	7	NULL	NULL	0	NULL	 liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination of detoxifying liver support systems with liver cell bioreactors may have additional benefits for the treatment of liver failure due to the replacement of known and unknown metabolic activities of the liver .
	manualset3
246555	1	425396	7	NULL	NULL	0	NULL	Combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination of intravitreal ranibizumab and laser photocoagulation for aggressive posterior retinopathy of prematurity .
	manualset3
246556	2	425396	7	NULL	NULL	0	NULL	intravitreal ranibizumab	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination of intravitreal ranibizumab and laser photocoagulation for aggressive posterior retinopathy of prematurity .
	manualset3
246557	3	425396	7	NULL	NULL	0	NULL	 laser photocoagulation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination of intravitreal ranibizumab and laser photocoagulation for aggressive posterior retinopathy of prematurity .
	manualset3
246558	4	425396	7	NULL	NULL	0	NULL	aggressive posterior retinopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination of intravitreal ranibizumab and laser photocoagulation for aggressive posterior retinopathy of prematurity .
	manualset3
246560	5	425396	7	NULL	NULL	0	NULL	prematurity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination of intravitreal ranibizumab and laser photocoagulation for aggressive posterior retinopathy of prematurity .
	manualset3
246561	1	425397	7	NULL	NULL	0	NULL	Combination therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination therapy with indacaterol plus tiotropium bromide improved lung function , dyspnoea , rescue medication use and general health status significantly more than tiotropium bromide alone in patients with moderate to severe COPD .
	manualset3
246562	2	425397	7	NULL	NULL	0	NULL	 indacaterol plus tiotropium bromide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination therapy with indacaterol plus tiotropium bromide improved lung function , dyspnoea , rescue medication use and general health status significantly more than tiotropium bromide alone in patients with moderate to severe COPD .
	manualset3
246563	3	425397	7	NULL	NULL	0	NULL	 lung function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination therapy with indacaterol plus tiotropium bromide improved lung function , dyspnoea , rescue medication use and general health status significantly more than tiotropium bromide alone in patients with moderate to severe COPD .
	manualset3
246564	4	425397	7	NULL	NULL	0	NULL	dyspnoea 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination therapy with indacaterol plus tiotropium bromide improved lung function , dyspnoea , rescue medication use and general health status significantly more than tiotropium bromide alone in patients with moderate to severe COPD .
	manualset3
246565	5	425397	7	NULL	NULL	0	NULL	medication use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination therapy with indacaterol plus tiotropium bromide improved lung function , dyspnoea , rescue medication use and general health status significantly more than tiotropium bromide alone in patients with moderate to severe COPD .
	manualset3
246566	6	425397	7	NULL	NULL	0	NULL	general health status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination therapy with indacaterol plus tiotropium bromide improved lung function , dyspnoea , rescue medication use and general health status significantly more than tiotropium bromide alone in patients with moderate to severe COPD .
	manualset3
246567	7	425397	7	NULL	NULL	0	NULL	tiotropium bromide 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination therapy with indacaterol plus tiotropium bromide improved lung function , dyspnoea , rescue medication use and general health status significantly more than tiotropium bromide alone in patients with moderate to severe COPD .
	manualset3
246568	8	425397	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination therapy with indacaterol plus tiotropium bromide improved lung function , dyspnoea , rescue medication use and general health status significantly more than tiotropium bromide alone in patients with moderate to severe COPD .
	manualset3
246569	9	425397	7	NULL	NULL	0	NULL	severe COPD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination therapy with indacaterol plus tiotropium bromide improved lung function , dyspnoea , rescue medication use and general health status significantly more than tiotropium bromide alone in patients with moderate to severe COPD .
	manualset3
246573	1	425398	7	NULL	NULL	0	NULL	Combination therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination therapy with intravesical bacillus Calmette-Guerin ( BCG ) plus interferon-alpha2b ( IFN-alpha2b ) for superficial transitional cell carcinoma ( TCC ) seems to be immune-dependent and activation of Th1 immune response is required for clinical efficacy .
	manualset3
246574	2	425398	7	NULL	NULL	NULL	NULL	intravesical bacillus Calmette-Guerin ( BCG ) plus interferon-alpha2b ( IFN-alpha2b )	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Combination therapy with intravesical bacillus Calmette-Guerin ( BCG ) plus interferon-alpha2b ( IFN-alpha2b ) for superficial transitional cell carcinoma ( TCC ) seems to be immune-dependent and activation of Th1 immune response is required for clinical efficacy .
	manualset3
246575	3	425398	7	NULL	NULL	0	NULL	 transitional cell carcinoma ( TCC ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination therapy with intravesical bacillus Calmette-Guerin ( BCG ) plus interferon-alpha2b ( IFN-alpha2b ) for superficial transitional cell carcinoma ( TCC ) seems to be immune-dependent and activation of Th1 immune response is required for clinical efficacy .
	manualset3
246576	4	425398	7	NULL	NULL	0	NULL	activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination therapy with intravesical bacillus Calmette-Guerin ( BCG ) plus interferon-alpha2b ( IFN-alpha2b ) for superficial transitional cell carcinoma ( TCC ) seems to be immune-dependent and activation of Th1 immune response is required for clinical efficacy .
	manualset3
246578	5	425398	7	NULL	NULL	0	NULL	Th1 immune response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination therapy with intravesical bacillus Calmette-Guerin ( BCG ) plus interferon-alpha2b ( IFN-alpha2b ) for superficial transitional cell carcinoma ( TCC ) seems to be immune-dependent and activation of Th1 immune response is required for clinical efficacy .
	manualset3
246580	6	425398	7	NULL	NULL	0	NULL	clinical efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination therapy with intravesical bacillus Calmette-Guerin ( BCG ) plus interferon-alpha2b ( IFN-alpha2b ) for superficial transitional cell carcinoma ( TCC ) seems to be immune-dependent and activation of Th1 immune response is required for clinical efficacy .
	manualset3
246582	1	425399	7	NULL	NULL	0	NULL	Combination therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination therapy with nicotinamide and tetracyclines for cicatricial pemphigoid : further support for its efficacy .
	manualset3
246583	2	425399	7	NULL	NULL	0	NULL	nicotinamide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination therapy with nicotinamide and tetracyclines for cicatricial pemphigoid : further support for its efficacy .
	manualset3
246584	3	425399	7	NULL	NULL	0	NULL	tetracyclines	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination therapy with nicotinamide and tetracyclines for cicatricial pemphigoid : further support for its efficacy .
	manualset3
246585	4	425399	7	NULL	NULL	0	NULL	cicatricial pemphigoid	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination therapy with nicotinamide and tetracyclines for cicatricial pemphigoid : further support for its efficacy .
	manualset3
246586	5	425399	7	NULL	NULL	0	NULL	support	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination therapy with nicotinamide and tetracyclines for cicatricial pemphigoid : further support for its efficacy .
	manualset3
246589	6	425399	7	NULL	NULL	0	NULL	 efficacy 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Combination therapy with nicotinamide and tetracyclines for cicatricial pemphigoid : further support for its efficacy .
	manualset3
246592	1	425400	7	NULL	NULL	0	NULL	Combinatorial peptide library binding 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Combinatorial peptide library binding of mammalian spermatozoa identifies a ligand ( HIPRT ) in the axin protein : putative identification of a sperm surface axin binding protein and intriguing developmental implications .
	manualset3
246593	2	425400	7	NULL	NULL	0	NULL	mammalian spermatozoa	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Combinatorial peptide library binding of mammalian spermatozoa identifies a ligand ( HIPRT ) in the axin protein : putative identification of a sperm surface axin binding protein and intriguing developmental implications .
	manualset3
246595	3	425400	7	NULL	NULL	0	NULL	ligand ( HIPRT )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Combinatorial peptide library binding of mammalian spermatozoa identifies a ligand ( HIPRT ) in the axin protein : putative identification of a sperm surface axin binding protein and intriguing developmental implications .
	manualset3
246596	4	425400	7	NULL	NULL	0	NULL	axin protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Combinatorial peptide library binding of mammalian spermatozoa identifies a ligand ( HIPRT ) in the axin protein : putative identification of a sperm surface axin binding protein and intriguing developmental implications .
	manualset3
246597	5	425400	7	NULL	NULL	0	NULL	putative identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Combinatorial peptide library binding of mammalian spermatozoa identifies a ligand ( HIPRT ) in the axin protein : putative identification of a sperm surface axin binding protein and intriguing developmental implications .
	manualset3
246598	6	425400	7	NULL	NULL	0	NULL	sperm surface axin binding protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Combinatorial peptide library binding of mammalian spermatozoa identifies a ligand ( HIPRT ) in the axin protein : putative identification of a sperm surface axin binding protein and intriguing developmental implications .
	manualset3
246602	7	425400	7	NULL	NULL	0	NULL	developmental implications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Combinatorial peptide library binding of mammalian spermatozoa identifies a ligand ( HIPRT ) in the axin protein : putative identification of a sperm surface axin binding protein and intriguing developmental implications .
	manualset3
246611	1	425401	7	NULL	NULL	0	NULL	Combined RNAi	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Combined RNAi and localization for functionally dissecting long noncoding RNAs .
	manualset3
246617	2	425401	7	NULL	NULL	NULL	NULL	localization	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Combined RNAi and localization for functionally dissecting long noncoding RNAs .
	manualset3
246618	3	425401	7	NULL	NULL	0	NULL	functionally dissecting long noncoding RNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Combined RNAi and localization for functionally dissecting long noncoding RNAs .
	manualset3
246630	1	425402	7	NULL	NULL	0	NULL	Combined chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Combined chemotherapy and sequential radiation therapy , hyperthermia or addition of intra-operative radiotherapy , have shown promising results , but no randomized studies have been published comparing the different treatment modalities .
	manualset3
246631	2	425402	7	NULL	NULL	0	NULL	sequential radiation therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Combined chemotherapy and sequential radiation therapy , hyperthermia or addition of intra-operative radiotherapy , have shown promising results , but no randomized studies have been published comparing the different treatment modalities .
	manualset3
246632	3	425402	7	NULL	NULL	0	NULL	hyperthermia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Combined chemotherapy and sequential radiation therapy , hyperthermia or addition of intra-operative radiotherapy , have shown promising results , but no randomized studies have been published comparing the different treatment modalities .
	manualset3
246633	4	425402	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Combined chemotherapy and sequential radiation therapy , hyperthermia or addition of intra-operative radiotherapy , have shown promising results , but no randomized studies have been published comparing the different treatment modalities .
	manualset3
246634	5	425402	7	NULL	NULL	0	NULL	intra-operative radiotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Combined chemotherapy and sequential radiation therapy , hyperthermia or addition of intra-operative radiotherapy , have shown promising results , but no randomized studies have been published comparing the different treatment modalities .
	manualset3
246635	6	425402	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Combined chemotherapy and sequential radiation therapy , hyperthermia or addition of intra-operative radiotherapy , have shown promising results , but no randomized studies have been published comparing the different treatment modalities .
	manualset3
246636	7	425402	7	NULL	NULL	0	NULL	no randomized studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Combined chemotherapy and sequential radiation therapy , hyperthermia or addition of intra-operative radiotherapy , have shown promising results , but no randomized studies have been published comparing the different treatment modalities .
	manualset3
246637	8	425402	7	NULL	NULL	0	NULL	different treatment modalities	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Combined chemotherapy and sequential radiation therapy , hyperthermia or addition of intra-operative radiotherapy , have shown promising results , but no randomized studies have been published comparing the different treatment modalities .
	manualset3
246640	1	425403	7	NULL	NULL	0	NULL	Combined chlorpromazine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Combined chlorpromazine and electroconvulsive therapy in mania .
	manualset3
246641	2	425403	7	NULL	NULL	0	NULL	electroconvulsive therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Combined chlorpromazine and electroconvulsive therapy in mania .
	manualset3
246642	3	425403	7	NULL	NULL	0	NULL	 mania	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Combined chlorpromazine and electroconvulsive therapy in mania .
	manualset3
246643	1	425404	7	NULL	NULL	0	NULL	previous study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Combined with the previous study using liver microsomes , these findings identify the limitations of in vitro covalent binding data for prospective prediction of hepatotoxicity for new drug candidates and highlight the need for a better understanding of the link between drug bioactivation , covalent adduct formation , and toxicity outcomes .
	manualset3
246644	2	425404	7	NULL	NULL	0	NULL	liver microsomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Combined with the previous study using liver microsomes , these findings identify the limitations of in vitro covalent binding data for prospective prediction of hepatotoxicity for new drug candidates and highlight the need for a better understanding of the link between drug bioactivation , covalent adduct formation , and toxicity outcomes .
	manualset3
246645	3	425404	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Combined with the previous study using liver microsomes , these findings identify the limitations of in vitro covalent binding data for prospective prediction of hepatotoxicity for new drug candidates and highlight the need for a better understanding of the link between drug bioactivation , covalent adduct formation , and toxicity outcomes .
	manualset3
246646	4	425404	7	NULL	NULL	0	NULL	limitations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Combined with the previous study using liver microsomes , these findings identify the limitations of in vitro covalent binding data for prospective prediction of hepatotoxicity for new drug candidates and highlight the need for a better understanding of the link between drug bioactivation , covalent adduct formation , and toxicity outcomes .
	manualset3
246647	5	425404	7	NULL	NULL	0	NULL	 in vitro covalent binding data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Combined with the previous study using liver microsomes , these findings identify the limitations of in vitro covalent binding data for prospective prediction of hepatotoxicity for new drug candidates and highlight the need for a better understanding of the link between drug bioactivation , covalent adduct formation , and toxicity outcomes .
	manualset3
246648	6	425404	7	NULL	NULL	0	NULL	prediction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Combined with the previous study using liver microsomes , these findings identify the limitations of in vitro covalent binding data for prospective prediction of hepatotoxicity for new drug candidates and highlight the need for a better understanding of the link between drug bioactivation , covalent adduct formation , and toxicity outcomes .
	manualset3
246649	7	425404	7	NULL	NULL	0	NULL	hepatotoxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Combined with the previous study using liver microsomes , these findings identify the limitations of in vitro covalent binding data for prospective prediction of hepatotoxicity for new drug candidates and highlight the need for a better understanding of the link between drug bioactivation , covalent adduct formation , and toxicity outcomes .
	manualset3
246650	8	425404	7	NULL	NULL	0	NULL	new drug candidates	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Combined with the previous study using liver microsomes , these findings identify the limitations of in vitro covalent binding data for prospective prediction of hepatotoxicity for new drug candidates and highlight the need for a better understanding of the link between drug bioactivation , covalent adduct formation , and toxicity outcomes .
	manualset3
246651	9	425404	7	NULL	NULL	0	NULL	understanding	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Combined with the previous study using liver microsomes , these findings identify the limitations of in vitro covalent binding data for prospective prediction of hepatotoxicity for new drug candidates and highlight the need for a better understanding of the link between drug bioactivation , covalent adduct formation , and toxicity outcomes .
	manualset3
246652	10	425404	7	NULL	NULL	0	NULL	drug bioactivation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Combined with the previous study using liver microsomes , these findings identify the limitations of in vitro covalent binding data for prospective prediction of hepatotoxicity for new drug candidates and highlight the need for a better understanding of the link between drug bioactivation , covalent adduct formation , and toxicity outcomes .
	manualset3
246653	11	425404	7	NULL	NULL	0	NULL	covalent adduct formation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Combined with the previous study using liver microsomes , these findings identify the limitations of in vitro covalent binding data for prospective prediction of hepatotoxicity for new drug candidates and highlight the need for a better understanding of the link between drug bioactivation , covalent adduct formation , and toxicity outcomes .
	manualset3
246654	12	425404	7	NULL	NULL	0	NULL	 toxicity outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Combined with the previous study using liver microsomes , these findings identify the limitations of in vitro covalent binding data for prospective prediction of hepatotoxicity for new drug candidates and highlight the need for a better understanding of the link between drug bioactivation , covalent adduct formation , and toxicity outcomes .
	manualset3
246656	1	425405	7	NULL	NULL	0	NULL	BBR3610	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining BBR3610 and PX-866 resulted in synergistic killing of cultured glioma cells and an extension of survival in an orthotopic xenograft animal model .
	manualset3
246657	2	425405	7	NULL	NULL	0	NULL	PX-866	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining BBR3610 and PX-866 resulted in synergistic killing of cultured glioma cells and an extension of survival in an orthotopic xenograft animal model .
	manualset3
246658	3	425405	7	NULL	NULL	0	NULL	synergistic killing 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining BBR3610 and PX-866 resulted in synergistic killing of cultured glioma cells and an extension of survival in an orthotopic xenograft animal model .
	manualset3
246662	4	425405	7	NULL	NULL	0	NULL	cultured glioma cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining BBR3610 and PX-866 resulted in synergistic killing of cultured glioma cells and an extension of survival in an orthotopic xenograft animal model .
	manualset3
246666	6	425405	7	NULL	NULL	0	NULL	extension	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining BBR3610 and PX-866 resulted in synergistic killing of cultured glioma cells and an extension of survival in an orthotopic xenograft animal model .
	manualset3
246667	7	425405	7	NULL	NULL	0	NULL	survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining BBR3610 and PX-866 resulted in synergistic killing of cultured glioma cells and an extension of survival in an orthotopic xenograft animal model .
	manualset3
246668	8	425405	7	NULL	NULL	0	NULL	orthotopic xenograft animal model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining BBR3610 and PX-866 resulted in synergistic killing of cultured glioma cells and an extension of survival in an orthotopic xenograft animal model .
	manualset3
246677	1	425406	7	NULL	NULL	0	NULL	PTX 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining PTX with either PD or LY had an additive effect on cell-growth inhibition .
	manualset3
246678	2	425406	7	NULL	NULL	0	NULL	PD	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining PTX with either PD or LY had an additive effect on cell-growth inhibition .
	manualset3
246679	3	425406	7	NULL	NULL	0	NULL	LY	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining PTX with either PD or LY had an additive effect on cell-growth inhibition .
	manualset3
246680	4	425406	7	NULL	NULL	NULL	NULL	additive effect 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Combining PTX with either PD or LY had an additive effect on cell-growth inhibition .
	manualset3
246682	5	425406	7	NULL	NULL	0	NULL	cell-growth inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining PTX with either PD or LY had an additive effect on cell-growth inhibition .
	manualset3
246689	1	425407	7	NULL	NULL	0	NULL	prognosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining with prognosis of subtypes of CHL i. e , LRHL ) NSHL ) MCHL , these data suggest that low ratio of T/B with high ratios of CD4 ( + ) / CD8 ( + ) and GrB ( + ) / TIA-1 ( + ) may represent biological markers predicting an unfavorable outcome of CHL subtypes .
	manualset3
246690	2	425407	7	NULL	NULL	0	NULL	subtypes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining with prognosis of subtypes of CHL i. e , LRHL ) NSHL ) MCHL , these data suggest that low ratio of T/B with high ratios of CD4 ( + ) / CD8 ( + ) and GrB ( + ) / TIA-1 ( + ) may represent biological markers predicting an unfavorable outcome of CHL subtypes .
	manualset3
246691	3	425407	7	NULL	NULL	0	NULL	 CHL	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining with prognosis of subtypes of CHL i. e , LRHL ) NSHL ) MCHL , these data suggest that low ratio of T/B with high ratios of CD4 ( + ) / CD8 ( + ) and GrB ( + ) / TIA-1 ( + ) may represent biological markers predicting an unfavorable outcome of CHL subtypes .
	manualset3
246692	4	425407	7	NULL	NULL	0	NULL	LRHL	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining with prognosis of subtypes of CHL i. e , LRHL ) NSHL ) MCHL , these data suggest that low ratio of T/B with high ratios of CD4 ( + ) / CD8 ( + ) and GrB ( + ) / TIA-1 ( + ) may represent biological markers predicting an unfavorable outcome of CHL subtypes .
	manualset3
246693	5	425407	7	NULL	NULL	0	NULL	NSHL	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining with prognosis of subtypes of CHL i. e , LRHL ) NSHL ) MCHL , these data suggest that low ratio of T/B with high ratios of CD4 ( + ) / CD8 ( + ) and GrB ( + ) / TIA-1 ( + ) may represent biological markers predicting an unfavorable outcome of CHL subtypes .
	manualset3
246694	6	425407	7	NULL	NULL	0	NULL	MCHL	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining with prognosis of subtypes of CHL i. e , LRHL ) NSHL ) MCHL , these data suggest that low ratio of T/B with high ratios of CD4 ( + ) / CD8 ( + ) and GrB ( + ) / TIA-1 ( + ) may represent biological markers predicting an unfavorable outcome of CHL subtypes .
	manualset3
246695	7	425407	7	NULL	NULL	0	NULL	data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining with prognosis of subtypes of CHL i. e , LRHL ) NSHL ) MCHL , these data suggest that low ratio of T/B with high ratios of CD4 ( + ) / CD8 ( + ) and GrB ( + ) / TIA-1 ( + ) may represent biological markers predicting an unfavorable outcome of CHL subtypes .
	manualset3
246696	8	425407	7	NULL	NULL	0	NULL	 low ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining with prognosis of subtypes of CHL i. e , LRHL ) NSHL ) MCHL , these data suggest that low ratio of T/B with high ratios of CD4 ( + ) / CD8 ( + ) and GrB ( + ) / TIA-1 ( + ) may represent biological markers predicting an unfavorable outcome of CHL subtypes .
	manualset3
246697	9	425407	7	NULL	NULL	0	NULL	 T/B	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining with prognosis of subtypes of CHL i. e , LRHL ) NSHL ) MCHL , these data suggest that low ratio of T/B with high ratios of CD4 ( + ) / CD8 ( + ) and GrB ( + ) / TIA-1 ( + ) may represent biological markers predicting an unfavorable outcome of CHL subtypes .
	manualset3
246698	10	425407	7	NULL	NULL	0	NULL	high ratios	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining with prognosis of subtypes of CHL i. e , LRHL ) NSHL ) MCHL , these data suggest that low ratio of T/B with high ratios of CD4 ( + ) / CD8 ( + ) and GrB ( + ) / TIA-1 ( + ) may represent biological markers predicting an unfavorable outcome of CHL subtypes .
	manualset3
246699	11	425407	7	NULL	NULL	0	NULL	CD4 ( + ) / CD8 ( + ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining with prognosis of subtypes of CHL i. e , LRHL ) NSHL ) MCHL , these data suggest that low ratio of T/B with high ratios of CD4 ( + ) / CD8 ( + ) and GrB ( + ) / TIA-1 ( + ) may represent biological markers predicting an unfavorable outcome of CHL subtypes .
	manualset3
246700	12	425407	7	NULL	NULL	0	NULL	 GrB ( + ) / TIA-1 ( + )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining with prognosis of subtypes of CHL i. e , LRHL ) NSHL ) MCHL , these data suggest that low ratio of T/B with high ratios of CD4 ( + ) / CD8 ( + ) and GrB ( + ) / TIA-1 ( + ) may represent biological markers predicting an unfavorable outcome of CHL subtypes .
	manualset3
246701	13	425407	7	NULL	NULL	0	NULL	biological markers	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining with prognosis of subtypes of CHL i. e , LRHL ) NSHL ) MCHL , these data suggest that low ratio of T/B with high ratios of CD4 ( + ) / CD8 ( + ) and GrB ( + ) / TIA-1 ( + ) may represent biological markers predicting an unfavorable outcome of CHL subtypes .
	manualset3
246702	14	425407	7	NULL	NULL	0	NULL	 unfavorable outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining with prognosis of subtypes of CHL i. e , LRHL ) NSHL ) MCHL , these data suggest that low ratio of T/B with high ratios of CD4 ( + ) / CD8 ( + ) and GrB ( + ) / TIA-1 ( + ) may represent biological markers predicting an unfavorable outcome of CHL subtypes .
	manualset3
246703	15	425407	7	NULL	NULL	0	NULL	CHL subtypes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Combining with prognosis of subtypes of CHL i. e , LRHL ) NSHL ) MCHL , these data suggest that low ratio of T/B with high ratios of CD4 ( + ) / CD8 ( + ) and GrB ( + ) / TIA-1 ( + ) may represent biological markers predicting an unfavorable outcome of CHL subtypes .
	manualset3
246704	1	425408	7	NULL	NULL	NULL	NULL	Combustion toxicology	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Combustion toxicology embraces the nature , the severity , and the time course of adverse effects produced upon exposure to fire-generated toxic species .
	manualset3
246707	2	425408	7	NULL	NULL	0	NULL	nature	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Combustion toxicology embraces the nature , the severity , and the time course of adverse effects produced upon exposure to fire-generated toxic species .
	manualset3
246708	3	425408	7	NULL	NULL	0	NULL	 severity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Combustion toxicology embraces the nature , the severity , and the time course of adverse effects produced upon exposure to fire-generated toxic species .
	manualset3
246709	4	425408	7	NULL	NULL	0	NULL	time course 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Combustion toxicology embraces the nature , the severity , and the time course of adverse effects produced upon exposure to fire-generated toxic species .
	manualset3
246710	5	425408	7	NULL	NULL	0	NULL	adverse effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Combustion toxicology embraces the nature , the severity , and the time course of adverse effects produced upon exposure to fire-generated toxic species .
	manualset3
246711	6	425408	7	NULL	NULL	0	NULL	exposure 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Combustion toxicology embraces the nature , the severity , and the time course of adverse effects produced upon exposure to fire-generated toxic species .
	manualset3
246713	7	425408	7	NULL	NULL	0	NULL	fire-generated toxic species 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Combustion toxicology embraces the nature , the severity , and the time course of adverse effects produced upon exposure to fire-generated toxic species .
	manualset3
246716	1	425409	7	NULL	NULL	0	NULL	 home	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Coming home from jail : the social and health consequences of community reentry for women , male adolescents , and their families and communities .
	manualset3
246717	2	425409	7	NULL	NULL	0	NULL	jail	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Coming home from jail : the social and health consequences of community reentry for women , male adolescents , and their families and communities .
	manualset3
246719	3	425409	7	NULL	NULL	0	NULL	social consequences	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Coming home from jail : the social and health consequences of community reentry for women , male adolescents , and their families and communities .
	manualset3
246720	4	425409	7	NULL	NULL	0	NULL	health consequences 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Coming home from jail : the social and health consequences of community reentry for women , male adolescents , and their families and communities .
	manualset3
246721	5	425409	7	NULL	NULL	0	NULL	community reentry	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Coming home from jail : the social and health consequences of community reentry for women , male adolescents , and their families and communities .
	manualset3
246723	6	425409	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Coming home from jail : the social and health consequences of community reentry for women , male adolescents , and their families and communities .
	manualset3
246724	7	425409	7	NULL	NULL	0	NULL	male adolescents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Coming home from jail : the social and health consequences of community reentry for women , male adolescents , and their families and communities .
	manualset3
246725	8	425409	7	NULL	NULL	0	NULL	families	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Coming home from jail : the social and health consequences of community reentry for women , male adolescents , and their families and communities .
	manualset3
246728	9	425409	7	NULL	NULL	0	NULL	communities	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Coming home from jail : the social and health consequences of community reentry for women , male adolescents , and their families and communities .
	manualset3
246729	1	425410	7	NULL	NULL	0	NULL	Comment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comment on `` Universality of quantum gravity corrections '' .
	manualset3
246730	2	425410	7	NULL	NULL	NULL	NULL	Universality quantum gravity corrections	PublicationOrCitation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Comment on `` Universality of quantum gravity corrections '' .
	manualset3
246733	1	425411	7	NULL	NULL	0	NULL	Comment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comment on the Nanoparticle Conclusions in Crts et al. ( 2008 ) , `` Exposure to diesel exhaust induces changes in EEG in human volunteers '' .
	manualset3
246735	2	425411	7	NULL	NULL	0	NULL	Nanoparticle Conclusions in Crts et al. ( 2008 )	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	Comment on the Nanoparticle Conclusions in Crts et al. ( 2008 ) , `` Exposure to diesel exhaust induces changes in EEG in human volunteers '' .
	manualset3
246737	3	425411	7	NULL	NULL	0	NULL	`` Exposure to diesel exhaust induces changes in EEG in human volunteers ''	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	Comment on the Nanoparticle Conclusions in Crts et al. ( 2008 ) , `` Exposure to diesel exhaust induces changes in EEG in human volunteers '' .
	manualset3
246739	1	425412	7	NULL	NULL	0	NULL	Commentary on paper	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Commentary on paper : `` A review of the mandibular and maxillary nerve supplies and their clinical relevance '' .
	manualset3
246741	2	425412	7	NULL	NULL	0	NULL	`` A review of the mandibular and maxillary nerve supplies and their clinical relevance ''	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	Commentary on paper : `` A review of the mandibular and maxillary nerve supplies and their clinical relevance '' .
	manualset3
246744	1	425413	7	NULL	NULL	0	NULL	Investigation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Investigation of antiviral activity of adamantan boron derivaties on pandemic influenza virus models ) .
	manualset3
246745	2	425413	7	NULL	NULL	0	NULL	antiviral activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Investigation of antiviral activity of adamantan boron derivaties on pandemic influenza virus models ) .
	manualset3
246746	3	425413	7	NULL	NULL	0	NULL	adamantan boron derivaties	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Investigation of antiviral activity of adamantan boron derivaties on pandemic influenza virus models ) .
	manualset3
246748	4	425413	7	NULL	NULL	0	NULL	pandemic influenza virus models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Investigation of antiviral activity of adamantan boron derivaties on pandemic influenza virus models ) .
	manualset3
246749	1	425414	7	NULL	NULL	NULL	NULL	Commentary	PublicationOrCitation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Commentary : Is capital the solution or the problem ?
	manualset3
246750	2	425414	7	NULL	NULL	0	NULL	Is capital the solution or the problem ?	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	Commentary : Is capital the solution or the problem ?
	manualset3
246755	1	425415	7	NULL	NULL	0	NULL	Commentary 	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	Commentary : once-daily aminoglycoside dosing : where are we now ?
	manualset3
246756	2	425415	7	NULL	NULL	0	NULL	once-daily aminoglycoside dosing : where are we now ?	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	Commentary : once-daily aminoglycoside dosing : where are we now ?
	manualset3
246759	1	425416	7	NULL	NULL	0	NULL	`` Personality traits and the classification of mental disorders	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	Commentary on `` Personality traits and the classification of mental disorders : Toward a more complete integration in DSM-5 and an empirical model of psychopathology '' .
	manualset3
246760	2	425416	7	NULL	NULL	0	NULL	complete integration 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Commentary on `` Personality traits and the classification of mental disorders : Toward a more complete integration in DSM-5 and an empirical model of psychopathology '' .
	manualset3
246763	3	425416	7	NULL	NULL	0	NULL	DSM-5	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Commentary on `` Personality traits and the classification of mental disorders : Toward a more complete integration in DSM-5 and an empirical model of psychopathology '' .
	manualset3
246764	4	425416	7	NULL	NULL	0	NULL	empirical model 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Commentary on `` Personality traits and the classification of mental disorders : Toward a more complete integration in DSM-5 and an empirical model of psychopathology '' .
	manualset3
246765	5	425416	7	NULL	NULL	0	NULL	psychopathology	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Commentary on `` Personality traits and the classification of mental disorders : Toward a more complete integration in DSM-5 and an empirical model of psychopathology '' .
	manualset3
246767	1	425417	7	NULL	NULL	0	NULL	T helper ( Th ) 2 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Committed T helper ( Th ) 2 cells exclusively expressed SOCS3 and production of Th2 cytokines , such as IL-4 and IL-5 , was much less dependent on CD28 costimulation compared with interferon gamma and IL-2 production in Th1 cells .
	manualset3
246769	2	425417	7	NULL	NULL	0	NULL	 SOCS3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Committed T helper ( Th ) 2 cells exclusively expressed SOCS3 and production of Th2 cytokines , such as IL-4 and IL-5 , was much less dependent on CD28 costimulation compared with interferon gamma and IL-2 production in Th1 cells .
	manualset3
246770	3	425417	7	NULL	NULL	0	NULL	production	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Committed T helper ( Th ) 2 cells exclusively expressed SOCS3 and production of Th2 cytokines , such as IL-4 and IL-5 , was much less dependent on CD28 costimulation compared with interferon gamma and IL-2 production in Th1 cells .
	manualset3
246771	4	425417	7	NULL	NULL	0	NULL	Th2 cytokines	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Committed T helper ( Th ) 2 cells exclusively expressed SOCS3 and production of Th2 cytokines , such as IL-4 and IL-5 , was much less dependent on CD28 costimulation compared with interferon gamma and IL-2 production in Th1 cells .
	manualset3
246772	5	425417	7	NULL	NULL	0	NULL	 IL-4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Committed T helper ( Th ) 2 cells exclusively expressed SOCS3 and production of Th2 cytokines , such as IL-4 and IL-5 , was much less dependent on CD28 costimulation compared with interferon gamma and IL-2 production in Th1 cells .
	manualset3
246774	6	425417	7	NULL	NULL	0	NULL	 IL-5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Committed T helper ( Th ) 2 cells exclusively expressed SOCS3 and production of Th2 cytokines , such as IL-4 and IL-5 , was much less dependent on CD28 costimulation compared with interferon gamma and IL-2 production in Th1 cells .
	manualset3
246775	7	425417	7	NULL	NULL	0	NULL	CD28 costimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Committed T helper ( Th ) 2 cells exclusively expressed SOCS3 and production of Th2 cytokines , such as IL-4 and IL-5 , was much less dependent on CD28 costimulation compared with interferon gamma and IL-2 production in Th1 cells .
	manualset3
246776	8	425417	7	NULL	NULL	0	NULL	interferon gamma	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Committed T helper ( Th ) 2 cells exclusively expressed SOCS3 and production of Th2 cytokines , such as IL-4 and IL-5 , was much less dependent on CD28 costimulation compared with interferon gamma and IL-2 production in Th1 cells .
	manualset3
246777	9	425417	7	NULL	NULL	0	NULL	IL-2 production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Committed T helper ( Th ) 2 cells exclusively expressed SOCS3 and production of Th2 cytokines , such as IL-4 and IL-5 , was much less dependent on CD28 costimulation compared with interferon gamma and IL-2 production in Th1 cells .
	manualset3
246778	10	425417	7	NULL	NULL	0	NULL	Th1 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Committed T helper ( Th ) 2 cells exclusively expressed SOCS3 and production of Th2 cytokines , such as IL-4 and IL-5 , was much less dependent on CD28 costimulation compared with interferon gamma and IL-2 production in Th1 cells .
	manualset3
246779	1	425418	7	NULL	NULL	0	NULL	Common chicory	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Common chicory is also known as blue sailors , succory , and coffeeweed .
	manualset3
246781	2	425418	7	NULL	NULL	0	NULL	blue sailors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Common chicory is also known as blue sailors , succory , and coffeeweed .
	manualset3
246782	3	425418	7	NULL	NULL	0	NULL	succory	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Common chicory is also known as blue sailors , succory , and coffeeweed .
	manualset3
246783	4	425418	7	NULL	NULL	0	NULL	coffeeweed	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Common chicory is also known as blue sailors , succory , and coffeeweed .
	manualset3
246784	1	425419	7	NULL	NULL	0	NULL	Common ground	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Common ground : a framework for selecting core quality measures for mental health and substance abuse care .
	manualset3
246785	2	425419	7	NULL	NULL	0	NULL	framework	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Common ground : a framework for selecting core quality measures for mental health and substance abuse care .
	manualset3
246786	3	425419	7	NULL	NULL	0	NULL	core quality measures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Common ground : a framework for selecting core quality measures for mental health and substance abuse care .
	manualset3
246788	4	425419	7	NULL	NULL	0	NULL	mental health	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Common ground : a framework for selecting core quality measures for mental health and substance abuse care .
	manualset3
246789	5	425419	7	NULL	NULL	0	NULL	substance abuse care	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Common ground : a framework for selecting core quality measures for mental health and substance abuse care .
	manualset3
246791	1	425420	7	NULL	NULL	0	NULL	roentgenological study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( A roentgenological study of the bladder neck ) .
	manualset3
246793	2	425420	7	NULL	NULL	0	NULL	bladder neck	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( A roentgenological study of the bladder neck ) .
	manualset3
246798	1	425421	7	NULL	NULL	0	NULL	neuropathological findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Common neuropathological findings of inferior frontal lobe dysfunction support both disinhibition and kindling models of TBI-induced aggression .
	manualset3
246799	2	425421	7	NULL	NULL	0	NULL	 inferior frontal lobe dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Common neuropathological findings of inferior frontal lobe dysfunction support both disinhibition and kindling models of TBI-induced aggression .
	manualset3
246800	3	425421	7	NULL	NULL	NULL	NULL	disinhibition	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Common neuropathological findings of inferior frontal lobe dysfunction support both disinhibition and kindling models of TBI-induced aggression .
	manualset3
246801	4	425421	7	NULL	NULL	0	NULL	kindling models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Common neuropathological findings of inferior frontal lobe dysfunction support both disinhibition and kindling models of TBI-induced aggression .
	manualset3
246802	5	425421	7	NULL	NULL	0	NULL	 TBI-induced aggression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Common neuropathological findings of inferior frontal lobe dysfunction support both disinhibition and kindling models of TBI-induced aggression .
	manualset3
246804	1	425422	7	NULL	NULL	0	NULL	Common repair pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Common repair pathways acting upon U.V. - and X-ray induced damage in diploid cells of Saccharomyces cerevisiae .
	manualset3
246807	2	425422	7	NULL	NULL	0	NULL	U.V. - induced damage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Common repair pathways acting upon U.V. - and X-ray induced damage in diploid cells of Saccharomyces cerevisiae .
	manualset3
246809	3	425422	7	NULL	NULL	0	NULL	 X-ray induced damage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Common repair pathways acting upon U.V. - and X-ray induced damage in diploid cells of Saccharomyces cerevisiae .
	manualset3
246810	4	425422	7	NULL	NULL	0	NULL	diploid cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Common repair pathways acting upon U.V. - and X-ray induced damage in diploid cells of Saccharomyces cerevisiae .
	manualset3
246811	5	425422	7	NULL	NULL	0	NULL	Saccharomyces cerevisiae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Common repair pathways acting upon U.V. - and X-ray induced damage in diploid cells of Saccharomyces cerevisiae .
	manualset3
246812	1	425423	7	NULL	NULL	0	NULL	quality	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Commonly , the quality of treatment plans is judged by a dose-volume histogram ( DVH ) in regards to satisfying a series of dose-volume constraints .
	manualset3
246813	2	425423	7	NULL	NULL	0	NULL	treatment plans	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Commonly , the quality of treatment plans is judged by a dose-volume histogram ( DVH ) in regards to satisfying a series of dose-volume constraints .
	manualset3
246814	3	425423	7	NULL	NULL	0	NULL	dose-volume histogram ( DVH )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Commonly , the quality of treatment plans is judged by a dose-volume histogram ( DVH ) in regards to satisfying a series of dose-volume constraints .
	manualset3
246815	4	425423	7	NULL	NULL	0	NULL	series	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Commonly , the quality of treatment plans is judged by a dose-volume histogram ( DVH ) in regards to satisfying a series of dose-volume constraints .
	manualset3
246817	5	425423	7	NULL	NULL	0	NULL	dose-volume constraints	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Commonly , the quality of treatment plans is judged by a dose-volume histogram ( DVH ) in regards to satisfying a series of dose-volume constraints .
	manualset3
246819	1	425424	7	NULL	NULL	0	NULL	Comorbid conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Comorbid conditions were malignancy in 30 % of patients , diabetes mellitus in 24 % , hypertension in 21 % , ischemic heart disease in 21 % , liver disease in 15 % , and chronic renal failure in 15 % .
	manualset3
246821	2	425424	7	NULL	NULL	0	NULL	30 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comorbid conditions were malignancy in 30 % of patients , diabetes mellitus in 24 % , hypertension in 21 % , ischemic heart disease in 21 % , liver disease in 15 % , and chronic renal failure in 15 % .
	manualset3
246822	3	425424	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comorbid conditions were malignancy in 30 % of patients , diabetes mellitus in 24 % , hypertension in 21 % , ischemic heart disease in 21 % , liver disease in 15 % , and chronic renal failure in 15 % .
	manualset3
246823	4	425424	7	NULL	NULL	0	NULL	diabetes mellitus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Comorbid conditions were malignancy in 30 % of patients , diabetes mellitus in 24 % , hypertension in 21 % , ischemic heart disease in 21 % , liver disease in 15 % , and chronic renal failure in 15 % .
	manualset3
246824	5	425424	7	NULL	NULL	0	NULL	24 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comorbid conditions were malignancy in 30 % of patients , diabetes mellitus in 24 % , hypertension in 21 % , ischemic heart disease in 21 % , liver disease in 15 % , and chronic renal failure in 15 % .
	manualset3
246825	6	425424	7	NULL	NULL	0	NULL	hypertension	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Comorbid conditions were malignancy in 30 % of patients , diabetes mellitus in 24 % , hypertension in 21 % , ischemic heart disease in 21 % , liver disease in 15 % , and chronic renal failure in 15 % .
	manualset3
246826	7	425424	7	NULL	NULL	0	NULL	 21 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comorbid conditions were malignancy in 30 % of patients , diabetes mellitus in 24 % , hypertension in 21 % , ischemic heart disease in 21 % , liver disease in 15 % , and chronic renal failure in 15 % .
	manualset3
246828	8	425424	7	NULL	NULL	0	NULL	ischemic heart disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Comorbid conditions were malignancy in 30 % of patients , diabetes mellitus in 24 % , hypertension in 21 % , ischemic heart disease in 21 % , liver disease in 15 % , and chronic renal failure in 15 % .
	manualset3
246830	9	425424	7	NULL	NULL	0	NULL	21 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comorbid conditions were malignancy in 30 % of patients , diabetes mellitus in 24 % , hypertension in 21 % , ischemic heart disease in 21 % , liver disease in 15 % , and chronic renal failure in 15 % .
	manualset3
246832	10	425424	7	NULL	NULL	0	NULL	liver disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Comorbid conditions were malignancy in 30 % of patients , diabetes mellitus in 24 % , hypertension in 21 % , ischemic heart disease in 21 % , liver disease in 15 % , and chronic renal failure in 15 % .
	manualset3
246833	11	425424	7	NULL	NULL	0	NULL	15 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comorbid conditions were malignancy in 30 % of patients , diabetes mellitus in 24 % , hypertension in 21 % , ischemic heart disease in 21 % , liver disease in 15 % , and chronic renal failure in 15 % .
	manualset3
246843	12	425424	7	NULL	NULL	0	NULL	chronic renal failure 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Comorbid conditions were malignancy in 30 % of patients , diabetes mellitus in 24 % , hypertension in 21 % , ischemic heart disease in 21 % , liver disease in 15 % , and chronic renal failure in 15 % .
	manualset3
246845	13	425424	7	NULL	NULL	0	NULL	15 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comorbid conditions were malignancy in 30 % of patients , diabetes mellitus in 24 % , hypertension in 21 % , ischemic heart disease in 21 % , liver disease in 15 % , and chronic renal failure in 15 % .
	manualset3
246848	1	425425	7	NULL	NULL	0	NULL	Comorbid disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Comorbid disorders may actually be clues to subtypes of PTSD .
	manualset3
246849	2	425425	7	NULL	NULL	0	NULL	subtypes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Comorbid disorders may actually be clues to subtypes of PTSD .
	manualset3
246851	3	425425	7	NULL	NULL	0	NULL	PTSD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Comorbid disorders may actually be clues to subtypes of PTSD .
	manualset3
246853	1	425426	7	NULL	NULL	0	NULL	Comorbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Comorbidity and disability in elderly Mexican and Mexican American adults : findings from Mexico and the southwestern United States .
	manualset3
246854	2	425426	7	NULL	NULL	0	NULL	disability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Comorbidity and disability in elderly Mexican and Mexican American adults : findings from Mexico and the southwestern United States .
	manualset3
246856	3	425426	7	NULL	NULL	0	NULL	 elderly Mexican adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comorbidity and disability in elderly Mexican and Mexican American adults : findings from Mexico and the southwestern United States .
	manualset3
246857	4	425426	7	NULL	NULL	0	NULL	Mexican American adults	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comorbidity and disability in elderly Mexican and Mexican American adults : findings from Mexico and the southwestern United States .
	manualset3
246858	5	425426	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Comorbidity and disability in elderly Mexican and Mexican American adults : findings from Mexico and the southwestern United States .
	manualset3
246860	6	425426	7	NULL	NULL	0	NULL	Mexico	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Comorbidity and disability in elderly Mexican and Mexican American adults : findings from Mexico and the southwestern United States .
	manualset3
246861	7	425426	7	NULL	NULL	0	NULL	southwestern United States	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Comorbidity and disability in elderly Mexican and Mexican American adults : findings from Mexico and the southwestern United States .
	manualset3
246863	1	425427	7	NULL	NULL	0	NULL	Compact bone fatigue damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Compact bone fatigue damage -- I. Residual strength and stiffness .
	manualset3
246864	2	425427	7	NULL	NULL	0	NULL	Residual strength	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Compact bone fatigue damage -- I. Residual strength and stiffness .
	manualset3
246865	3	425427	7	NULL	NULL	0	NULL	stiffness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Compact bone fatigue damage -- I. Residual strength and stiffness .
	manualset3
246870	1	425428	7	NULL	NULL	0	NULL	Comparable incremental amino acid areas 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparable incremental amino acid areas after both meals suggested that the total amount of amino acids absorbed was not influenced by processing .
	manualset3
246871	2	425428	7	NULL	NULL	0	NULL	meals	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparable incremental amino acid areas after both meals suggested that the total amount of amino acids absorbed was not influenced by processing .
	manualset3
246872	3	425428	7	NULL	NULL	0	NULL	total amount 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparable incremental amino acid areas after both meals suggested that the total amount of amino acids absorbed was not influenced by processing .
	manualset3
246873	4	425428	7	NULL	NULL	0	NULL	amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparable incremental amino acid areas after both meals suggested that the total amount of amino acids absorbed was not influenced by processing .
	manualset3
246876	1	425429	7	NULL	NULL	0	NULL	Investigation 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Investigation on occupational risks of welding workers in a factory ) .
	manualset3
246877	2	425429	7	NULL	NULL	0	NULL	occupational risks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Investigation on occupational risks of welding workers in a factory ) .
	manualset3
246879	3	425429	7	NULL	NULL	0	NULL	welding workers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Investigation on occupational risks of welding workers in a factory ) .
	manualset3
246881	4	425429	7	NULL	NULL	0	NULL	factory	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( Investigation on occupational risks of welding workers in a factory ) .
	manualset3
246883	1	425430	7	NULL	NULL	0	NULL	Comparative analysis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative analysis of 16S rRNA gene sequences showed that the novel strain was most closely related to genera within the family Nocardiopsaceae , but formed a separate lineage .
	manualset3
246884	2	425430	7	NULL	NULL	0	NULL	16S rRNA gene sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative analysis of 16S rRNA gene sequences showed that the novel strain was most closely related to genera within the family Nocardiopsaceae , but formed a separate lineage .
	manualset3
246885	3	425430	7	NULL	NULL	0	NULL	novel strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative analysis of 16S rRNA gene sequences showed that the novel strain was most closely related to genera within the family Nocardiopsaceae , but formed a separate lineage .
	manualset3
246886	4	425430	7	NULL	NULL	0	NULL	 family Nocardiopsaceae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative analysis of 16S rRNA gene sequences showed that the novel strain was most closely related to genera within the family Nocardiopsaceae , but formed a separate lineage .
	manualset3
246887	5	425430	7	NULL	NULL	0	NULL	separate lineage	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative analysis of 16S rRNA gene sequences showed that the novel strain was most closely related to genera within the family Nocardiopsaceae , but formed a separate lineage .
	manualset3
247477	1	425431	7	NULL	NULL	0	NULL	Comparative analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative analysis of the metabolite profiles in both rat strains after exposure to KC500 showed higher formation ratios of several dihydroxy PCB metabolites in the liver of Gunn rats ; major metabolites are the catechols from 2 , 5 , 3 ' , 4 ' - tetraCB , CB101 , 2 , 3 , 6 , 3 ' , 4 ' - pentaCB , and 2 , 3 , 6 , 2 ' , 4 ' , 5 ' - pentaCB .
	manualset3
247478	2	425431	7	NULL	NULL	0	NULL	 metabolite profiles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative analysis of the metabolite profiles in both rat strains after exposure to KC500 showed higher formation ratios of several dihydroxy PCB metabolites in the liver of Gunn rats ; major metabolites are the catechols from 2 , 5 , 3 ' , 4 ' - tetraCB , CB101 , 2 , 3 , 6 , 3 ' , 4 ' - pentaCB , and 2 , 3 , 6 , 2 ' , 4 ' , 5 ' - pentaCB .
	manualset3
247479	3	425431	7	NULL	NULL	0	NULL	rat strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative analysis of the metabolite profiles in both rat strains after exposure to KC500 showed higher formation ratios of several dihydroxy PCB metabolites in the liver of Gunn rats ; major metabolites are the catechols from 2 , 5 , 3 ' , 4 ' - tetraCB , CB101 , 2 , 3 , 6 , 3 ' , 4 ' - pentaCB , and 2 , 3 , 6 , 2 ' , 4 ' , 5 ' - pentaCB .
	manualset3
247480	4	425431	7	NULL	NULL	0	NULL	 exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative analysis of the metabolite profiles in both rat strains after exposure to KC500 showed higher formation ratios of several dihydroxy PCB metabolites in the liver of Gunn rats ; major metabolites are the catechols from 2 , 5 , 3 ' , 4 ' - tetraCB , CB101 , 2 , 3 , 6 , 3 ' , 4 ' - pentaCB , and 2 , 3 , 6 , 2 ' , 4 ' , 5 ' - pentaCB .
	manualset3
247481	5	425431	7	NULL	NULL	0	NULL	KC500	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative analysis of the metabolite profiles in both rat strains after exposure to KC500 showed higher formation ratios of several dihydroxy PCB metabolites in the liver of Gunn rats ; major metabolites are the catechols from 2 , 5 , 3 ' , 4 ' - tetraCB , CB101 , 2 , 3 , 6 , 3 ' , 4 ' - pentaCB , and 2 , 3 , 6 , 2 ' , 4 ' , 5 ' - pentaCB .
	manualset3
247482	6	425431	7	NULL	NULL	0	NULL	formation ratios	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative analysis of the metabolite profiles in both rat strains after exposure to KC500 showed higher formation ratios of several dihydroxy PCB metabolites in the liver of Gunn rats ; major metabolites are the catechols from 2 , 5 , 3 ' , 4 ' - tetraCB , CB101 , 2 , 3 , 6 , 3 ' , 4 ' - pentaCB , and 2 , 3 , 6 , 2 ' , 4 ' , 5 ' - pentaCB .
	manualset3
247483	7	425431	7	NULL	NULL	0	NULL	dihydroxy PCB metabolites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative analysis of the metabolite profiles in both rat strains after exposure to KC500 showed higher formation ratios of several dihydroxy PCB metabolites in the liver of Gunn rats ; major metabolites are the catechols from 2 , 5 , 3 ' , 4 ' - tetraCB , CB101 , 2 , 3 , 6 , 3 ' , 4 ' - pentaCB , and 2 , 3 , 6 , 2 ' , 4 ' , 5 ' - pentaCB .
	manualset3
247484	8	425431	7	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative analysis of the metabolite profiles in both rat strains after exposure to KC500 showed higher formation ratios of several dihydroxy PCB metabolites in the liver of Gunn rats ; major metabolites are the catechols from 2 , 5 , 3 ' , 4 ' - tetraCB , CB101 , 2 , 3 , 6 , 3 ' , 4 ' - pentaCB , and 2 , 3 , 6 , 2 ' , 4 ' , 5 ' - pentaCB .
	manualset3
247485	9	425431	7	NULL	NULL	0	NULL	Gunn rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative analysis of the metabolite profiles in both rat strains after exposure to KC500 showed higher formation ratios of several dihydroxy PCB metabolites in the liver of Gunn rats ; major metabolites are the catechols from 2 , 5 , 3 ' , 4 ' - tetraCB , CB101 , 2 , 3 , 6 , 3 ' , 4 ' - pentaCB , and 2 , 3 , 6 , 2 ' , 4 ' , 5 ' - pentaCB .
	manualset3
247486	10	425431	7	NULL	NULL	0	NULL	major metabolites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative analysis of the metabolite profiles in both rat strains after exposure to KC500 showed higher formation ratios of several dihydroxy PCB metabolites in the liver of Gunn rats ; major metabolites are the catechols from 2 , 5 , 3 ' , 4 ' - tetraCB , CB101 , 2 , 3 , 6 , 3 ' , 4 ' - pentaCB , and 2 , 3 , 6 , 2 ' , 4 ' , 5 ' - pentaCB .
	manualset3
247487	11	425431	7	NULL	NULL	0	NULL	catechols	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative analysis of the metabolite profiles in both rat strains after exposure to KC500 showed higher formation ratios of several dihydroxy PCB metabolites in the liver of Gunn rats ; major metabolites are the catechols from 2 , 5 , 3 ' , 4 ' - tetraCB , CB101 , 2 , 3 , 6 , 3 ' , 4 ' - pentaCB , and 2 , 3 , 6 , 2 ' , 4 ' , 5 ' - pentaCB .
	manualset3
247488	12	425431	7	NULL	NULL	0	NULL	2 , 5 , 3 ' , 4 ' - tetraCB	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative analysis of the metabolite profiles in both rat strains after exposure to KC500 showed higher formation ratios of several dihydroxy PCB metabolites in the liver of Gunn rats ; major metabolites are the catechols from 2 , 5 , 3 ' , 4 ' - tetraCB , CB101 , 2 , 3 , 6 , 3 ' , 4 ' - pentaCB , and 2 , 3 , 6 , 2 ' , 4 ' , 5 ' - pentaCB .
	manualset3
247489	13	425431	7	NULL	NULL	0	NULL	CB101 , 2 , 3 , 6 , 3 ' , 4 ' - pentaCB	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative analysis of the metabolite profiles in both rat strains after exposure to KC500 showed higher formation ratios of several dihydroxy PCB metabolites in the liver of Gunn rats ; major metabolites are the catechols from 2 , 5 , 3 ' , 4 ' - tetraCB , CB101 , 2 , 3 , 6 , 3 ' , 4 ' - pentaCB , and 2 , 3 , 6 , 2 ' , 4 ' , 5 ' - pentaCB .
	manualset3
247490	14	425431	7	NULL	NULL	0	NULL	 2 , 3 , 6 , 2 ' , 4 ' , 5 ' - pentaCB	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative analysis of the metabolite profiles in both rat strains after exposure to KC500 showed higher formation ratios of several dihydroxy PCB metabolites in the liver of Gunn rats ; major metabolites are the catechols from 2 , 5 , 3 ' , 4 ' - tetraCB , CB101 , 2 , 3 , 6 , 3 ' , 4 ' - pentaCB , and 2 , 3 , 6 , 2 ' , 4 ' , 5 ' - pentaCB .
	manualset3
247491	1	425432	7	NULL	NULL	0	NULL	Comparative effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative effects of holotoxin and its ADP-ribosylating S1 subunit .
	manualset3
247492	2	425432	7	NULL	NULL	0	NULL	holotoxin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative effects of holotoxin and its ADP-ribosylating S1 subunit .
	manualset3
247493	3	425432	7	NULL	NULL	0	NULL	ADP-ribosylating S1 subunit	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative effects of holotoxin and its ADP-ribosylating S1 subunit .
	manualset3
247494	1	425433	7	NULL	NULL	0	NULL	Comparative efficiency	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative efficiency of different diluents for preservation of bull and buffalo bull semen .
	manualset3
247495	2	425433	7	NULL	NULL	0	NULL	different diluents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative efficiency of different diluents for preservation of bull and buffalo bull semen .
	manualset3
247496	3	425433	7	NULL	NULL	0	NULL	preservation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative efficiency of different diluents for preservation of bull and buffalo bull semen .
	manualset3
247497	4	425433	7	NULL	NULL	0	NULL	bull	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative efficiency of different diluents for preservation of bull and buffalo bull semen .
	manualset3
247498	5	425433	7	NULL	NULL	0	NULL	buffalo bull semen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative efficiency of different diluents for preservation of bull and buffalo bull semen .
	manualset3
247499	1	425434	7	NULL	NULL	0	NULL	Comparative electron microscopic studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative electron microscopic studies on juvenile and adult bovine leukosis .
	manualset3
247500	2	425434	7	NULL	NULL	0	NULL	juvenile leukosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative electron microscopic studies on juvenile and adult bovine leukosis .
	manualset3
247501	3	425434	7	NULL	NULL	0	NULL	adult bovine leukosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative electron microscopic studies on juvenile and adult bovine leukosis .
	manualset3
247502	1	425435	7	NULL	NULL	0	NULL	Comparative field evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative field evaluation of residual-sprayed deltamethrin WG and deltamethrin WP for the control of malaria in Pahang , Malaysia .
	manualset3
247503	2	425435	7	NULL	NULL	0	NULL	 residual-sprayed deltamethrin WG 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative field evaluation of residual-sprayed deltamethrin WG and deltamethrin WP for the control of malaria in Pahang , Malaysia .
	manualset3
247504	3	425435	7	NULL	NULL	0	NULL	 deltamethrin WP	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative field evaluation of residual-sprayed deltamethrin WG and deltamethrin WP for the control of malaria in Pahang , Malaysia .
	manualset3
247505	4	425435	7	NULL	NULL	0	NULL	control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative field evaluation of residual-sprayed deltamethrin WG and deltamethrin WP for the control of malaria in Pahang , Malaysia .
	manualset3
247506	5	425435	7	NULL	NULL	0	NULL	malaria	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative field evaluation of residual-sprayed deltamethrin WG and deltamethrin WP for the control of malaria in Pahang , Malaysia .
	manualset3
247507	6	425435	7	NULL	NULL	0	NULL	Pahang	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative field evaluation of residual-sprayed deltamethrin WG and deltamethrin WP for the control of malaria in Pahang , Malaysia .
	manualset3
247508	7	425435	7	NULL	NULL	0	NULL	Malaysia	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative field evaluation of residual-sprayed deltamethrin WG and deltamethrin WP for the control of malaria in Pahang , Malaysia .
	manualset3
247509	1	425436	7	NULL	NULL	0	NULL	Comparative in-vitro study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative in-vitro study with polyethylene and ceramic liners .
	manualset3
247510	2	425436	7	NULL	NULL	0	NULL	polyethylene liners	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative in-vitro study with polyethylene and ceramic liners .
	manualset3
247511	3	425436	7	NULL	NULL	0	NULL	ceramic liners	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative in-vitro study with polyethylene and ceramic liners .
	manualset3
247512	1	425437	7	NULL	NULL	0	NULL	 in vitro evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative in vitro and in vivo evaluation of three tablet formulations of amiodarone in healthy subjects .
	manualset3
247513	2	425437	7	NULL	NULL	0	NULL	 in vivo evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative in vitro and in vivo evaluation of three tablet formulations of amiodarone in healthy subjects .
	manualset3
247514	3	425437	7	NULL	NULL	0	NULL	three tablet formulations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative in vitro and in vivo evaluation of three tablet formulations of amiodarone in healthy subjects .
	manualset3
247515	4	425437	7	NULL	NULL	0	NULL	amiodarone 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative in vitro and in vivo evaluation of three tablet formulations of amiodarone in healthy subjects .
	manualset3
247516	5	425437	7	NULL	NULL	0	NULL	healthy subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative in vitro and in vivo evaluation of three tablet formulations of amiodarone in healthy subjects .
	manualset3
247517	1	425438	7	NULL	NULL	0	NULL	Comparative mapping	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative mapping of opioid receptors and enkephalin immunoreactive nerve terminals in the rat hippocampus .
	manualset3
247518	2	425438	7	NULL	NULL	0	NULL	opioid receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative mapping of opioid receptors and enkephalin immunoreactive nerve terminals in the rat hippocampus .
	manualset3
247519	3	425438	7	NULL	NULL	0	NULL	enkephalin immunoreactive nerve terminals	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative mapping of opioid receptors and enkephalin immunoreactive nerve terminals in the rat hippocampus .
	manualset3
247520	4	425438	7	NULL	NULL	0	NULL	 rat hippocampus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative mapping of opioid receptors and enkephalin immunoreactive nerve terminals in the rat hippocampus .
	manualset3
247521	1	425439	7	NULL	NULL	NULL	NULL	Involvement	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Involvement of H1 histone phosphorylation in chromosome condensation at mitosis ) .
	manualset3
247522	2	425439	7	NULL	NULL	0	NULL	H1 histone phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Involvement of H1 histone phosphorylation in chromosome condensation at mitosis ) .
	manualset3
247523	3	425439	7	NULL	NULL	0	NULL	chromosome condensation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Involvement of H1 histone phosphorylation in chromosome condensation at mitosis ) .
	manualset3
247524	4	425439	7	NULL	NULL	0	NULL	mitosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Involvement of H1 histone phosphorylation in chromosome condensation at mitosis ) .
	manualset3
247525	1	425440	7	NULL	NULL	0	NULL	Comparative safety evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative safety evaluation of non-narcotic analgesics .
	manualset3
247526	2	425440	7	NULL	NULL	0	NULL	non-narcotic analgesics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative safety evaluation of non-narcotic analgesics .
	manualset3
247527	1	425441	7	NULL	NULL	0	NULL	Comparative studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative studies of the effects of estradiol , progesterone , testosterone , cholesterol , and megestrol on juvenile chickens were carried out to determine their effects on bone and other physiological parameters .
	manualset3
247528	2	425441	7	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative studies of the effects of estradiol , progesterone , testosterone , cholesterol , and megestrol on juvenile chickens were carried out to determine their effects on bone and other physiological parameters .
	manualset3
247529	3	425441	7	NULL	NULL	0	NULL	estradiol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative studies of the effects of estradiol , progesterone , testosterone , cholesterol , and megestrol on juvenile chickens were carried out to determine their effects on bone and other physiological parameters .
	manualset3
247530	4	425441	7	NULL	NULL	0	NULL	progesterone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative studies of the effects of estradiol , progesterone , testosterone , cholesterol , and megestrol on juvenile chickens were carried out to determine their effects on bone and other physiological parameters .
	manualset3
247531	5	425441	7	NULL	NULL	0	NULL	 testosterone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative studies of the effects of estradiol , progesterone , testosterone , cholesterol , and megestrol on juvenile chickens were carried out to determine their effects on bone and other physiological parameters .
	manualset3
247532	6	425441	7	NULL	NULL	0	NULL	cholesterol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative studies of the effects of estradiol , progesterone , testosterone , cholesterol , and megestrol on juvenile chickens were carried out to determine their effects on bone and other physiological parameters .
	manualset3
247533	7	425441	7	NULL	NULL	0	NULL	megestrol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative studies of the effects of estradiol , progesterone , testosterone , cholesterol , and megestrol on juvenile chickens were carried out to determine their effects on bone and other physiological parameters .
	manualset3
247534	8	425441	7	NULL	NULL	0	NULL	 juvenile chickens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative studies of the effects of estradiol , progesterone , testosterone , cholesterol , and megestrol on juvenile chickens were carried out to determine their effects on bone and other physiological parameters .
	manualset3
247535	9	425441	7	NULL	NULL	0	NULL	effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative studies of the effects of estradiol , progesterone , testosterone , cholesterol , and megestrol on juvenile chickens were carried out to determine their effects on bone and other physiological parameters .
	manualset3
247536	10	425441	7	NULL	NULL	0	NULL	bone	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative studies of the effects of estradiol , progesterone , testosterone , cholesterol , and megestrol on juvenile chickens were carried out to determine their effects on bone and other physiological parameters .
	manualset3
247537	11	425441	7	NULL	NULL	0	NULL	physiological parameters	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative studies of the effects of estradiol , progesterone , testosterone , cholesterol , and megestrol on juvenile chickens were carried out to determine their effects on bone and other physiological parameters .
	manualset3
247538	1	425442	7	NULL	NULL	0	NULL	Comparative study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative study of the efficacy of gentamicin sulfate and cefoperazone in free and liposome-entrapped forms showed that immobilization of the antibiotics in phospholipid vesicles provided a 2-fold increase of their efficacy .
	manualset3
247539	2	425442	7	NULL	NULL	0	NULL	efficacy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative study of the efficacy of gentamicin sulfate and cefoperazone in free and liposome-entrapped forms showed that immobilization of the antibiotics in phospholipid vesicles provided a 2-fold increase of their efficacy .
	manualset3
247540	3	425442	7	NULL	NULL	0	NULL	gentamicin sulfate	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative study of the efficacy of gentamicin sulfate and cefoperazone in free and liposome-entrapped forms showed that immobilization of the antibiotics in phospholipid vesicles provided a 2-fold increase of their efficacy .
	manualset3
247541	4	425442	7	NULL	NULL	0	NULL	cefoperazone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative study of the efficacy of gentamicin sulfate and cefoperazone in free and liposome-entrapped forms showed that immobilization of the antibiotics in phospholipid vesicles provided a 2-fold increase of their efficacy .
	manualset3
247542	5	425442	7	NULL	NULL	0	NULL	liposome-entrapped forms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative study of the efficacy of gentamicin sulfate and cefoperazone in free and liposome-entrapped forms showed that immobilization of the antibiotics in phospholipid vesicles provided a 2-fold increase of their efficacy .
	manualset3
247543	6	425442	7	NULL	NULL	0	NULL	 immobilization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative study of the efficacy of gentamicin sulfate and cefoperazone in free and liposome-entrapped forms showed that immobilization of the antibiotics in phospholipid vesicles provided a 2-fold increase of their efficacy .
	manualset3
247544	7	425442	7	NULL	NULL	0	NULL	antibiotics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative study of the efficacy of gentamicin sulfate and cefoperazone in free and liposome-entrapped forms showed that immobilization of the antibiotics in phospholipid vesicles provided a 2-fold increase of their efficacy .
	manualset3
247545	8	425442	7	NULL	NULL	0	NULL	phospholipid vesicles	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative study of the efficacy of gentamicin sulfate and cefoperazone in free and liposome-entrapped forms showed that immobilization of the antibiotics in phospholipid vesicles provided a 2-fold increase of their efficacy .
	manualset3
247546	9	425442	7	NULL	NULL	0	NULL	2-fold increase	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative study of the efficacy of gentamicin sulfate and cefoperazone in free and liposome-entrapped forms showed that immobilization of the antibiotics in phospholipid vesicles provided a 2-fold increase of their efficacy .
	manualset3
247547	10	425442	7	NULL	NULL	0	NULL	efficacy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative study of the efficacy of gentamicin sulfate and cefoperazone in free and liposome-entrapped forms showed that immobilization of the antibiotics in phospholipid vesicles provided a 2-fold increase of their efficacy .
	manualset3
247548	11	425442	7	NULL	NULL	0	NULL	free forms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative study of the efficacy of gentamicin sulfate and cefoperazone in free and liposome-entrapped forms showed that immobilization of the antibiotics in phospholipid vesicles provided a 2-fold increase of their efficacy .
	manualset3
247549	1	425443	7	NULL	NULL	0	NULL	Comparative study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative study to the man ( author 's transl ) ) .
	manualset3
247550	2	425443	7	NULL	NULL	0	NULL	 man	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative study to the man ( author 's transl ) ) .
	manualset3
247551	3	425443	7	NULL	NULL	0	NULL	author 's transl 	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative study to the man ( author 's transl ) ) .
	manualset3
247552	1	425444	7	NULL	NULL	0	NULL	Comparative toxicogenomic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative toxicogenomic analysis revealed that both adult and larval fins respond to TCDD during regeneration with misexpression of Wnt signaling pathway members and Wnt target genes .
	manualset3
247553	2	425444	7	NULL	NULL	NULL	NULL	adult fins	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Comparative toxicogenomic analysis revealed that both adult and larval fins respond to TCDD during regeneration with misexpression of Wnt signaling pathway members and Wnt target genes .
	manualset3
247554	3	425444	7	NULL	NULL	NULL	NULL	larval fins	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Comparative toxicogenomic analysis revealed that both adult and larval fins respond to TCDD during regeneration with misexpression of Wnt signaling pathway members and Wnt target genes .
	manualset3
247555	4	425444	7	NULL	NULL	NULL	NULL	TCDD	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Comparative toxicogenomic analysis revealed that both adult and larval fins respond to TCDD during regeneration with misexpression of Wnt signaling pathway members and Wnt target genes .
	manualset3
247556	5	425444	7	NULL	NULL	0	NULL	 regeneration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative toxicogenomic analysis revealed that both adult and larval fins respond to TCDD during regeneration with misexpression of Wnt signaling pathway members and Wnt target genes .
	manualset3
247557	6	425444	7	NULL	NULL	0	NULL	misexpression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative toxicogenomic analysis revealed that both adult and larval fins respond to TCDD during regeneration with misexpression of Wnt signaling pathway members and Wnt target genes .
	manualset3
247558	7	425444	7	NULL	NULL	0	NULL	Wnt signaling pathway members	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative toxicogenomic analysis revealed that both adult and larval fins respond to TCDD during regeneration with misexpression of Wnt signaling pathway members and Wnt target genes .
	manualset3
247559	8	425444	7	NULL	NULL	0	NULL	Wnt target genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparative toxicogenomic analysis revealed that both adult and larval fins respond to TCDD during regeneration with misexpression of Wnt signaling pathway members and Wnt target genes .
	manualset3
247560	1	425445	7	NULL	NULL	0	NULL	bacteriological culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to bacteriological culture the combination of IMS and m-PCR resulted a faster method for the detection and identification of Salmonella at genus and serovar level by using of universal and specific primers .
	manualset3
247561	2	425445	7	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to bacteriological culture the combination of IMS and m-PCR resulted a faster method for the detection and identification of Salmonella at genus and serovar level by using of universal and specific primers .
	manualset3
247562	3	425445	7	NULL	NULL	0	NULL	 IMS	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to bacteriological culture the combination of IMS and m-PCR resulted a faster method for the detection and identification of Salmonella at genus and serovar level by using of universal and specific primers .
	manualset3
247563	4	425445	7	NULL	NULL	0	NULL	 m-PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to bacteriological culture the combination of IMS and m-PCR resulted a faster method for the detection and identification of Salmonella at genus and serovar level by using of universal and specific primers .
	manualset3
247564	5	425445	7	NULL	NULL	0	NULL	faster method	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to bacteriological culture the combination of IMS and m-PCR resulted a faster method for the detection and identification of Salmonella at genus and serovar level by using of universal and specific primers .
	manualset3
247565	6	425445	7	NULL	NULL	0	NULL	detection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to bacteriological culture the combination of IMS and m-PCR resulted a faster method for the detection and identification of Salmonella at genus and serovar level by using of universal and specific primers .
	manualset3
247566	7	425445	7	NULL	NULL	0	NULL	identification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to bacteriological culture the combination of IMS and m-PCR resulted a faster method for the detection and identification of Salmonella at genus and serovar level by using of universal and specific primers .
	manualset3
247567	8	425445	7	NULL	NULL	0	NULL	Salmonella	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to bacteriological culture the combination of IMS and m-PCR resulted a faster method for the detection and identification of Salmonella at genus and serovar level by using of universal and specific primers .
	manualset3
247568	9	425445	7	NULL	NULL	NULL	NULL	genus level	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Compared to bacteriological culture the combination of IMS and m-PCR resulted a faster method for the detection and identification of Salmonella at genus and serovar level by using of universal and specific primers .
	manualset3
247569	10	425445	7	NULL	NULL	0	NULL	serovar level	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to bacteriological culture the combination of IMS and m-PCR resulted a faster method for the detection and identification of Salmonella at genus and serovar level by using of universal and specific primers .
	manualset3
247570	11	425445	7	NULL	NULL	0	NULL	universal primers	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to bacteriological culture the combination of IMS and m-PCR resulted a faster method for the detection and identification of Salmonella at genus and serovar level by using of universal and specific primers .
	manualset3
247571	12	425445	7	NULL	NULL	0	NULL	specific primers	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to bacteriological culture the combination of IMS and m-PCR resulted a faster method for the detection and identification of Salmonella at genus and serovar level by using of universal and specific primers .
	manualset3
247572	1	425446	7	NULL	NULL	0	NULL	 controls	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to controls , PD patients were impaired in all conditions and the severity of the deficit was significantly correlated with that observed in tests of executive functions .
	manualset3
247573	2	425446	7	NULL	NULL	0	NULL	PD patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to controls , PD patients were impaired in all conditions and the severity of the deficit was significantly correlated with that observed in tests of executive functions .
	manualset3
247574	3	425446	7	NULL	NULL	0	NULL	all conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to controls , PD patients were impaired in all conditions and the severity of the deficit was significantly correlated with that observed in tests of executive functions .
	manualset3
247575	4	425446	7	NULL	NULL	0	NULL	severity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to controls , PD patients were impaired in all conditions and the severity of the deficit was significantly correlated with that observed in tests of executive functions .
	manualset3
247576	5	425446	7	NULL	NULL	0	NULL	deficit 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to controls , PD patients were impaired in all conditions and the severity of the deficit was significantly correlated with that observed in tests of executive functions .
	manualset3
247577	6	425446	7	NULL	NULL	0	NULL	 tests 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to controls , PD patients were impaired in all conditions and the severity of the deficit was significantly correlated with that observed in tests of executive functions .
	manualset3
247578	7	425446	7	NULL	NULL	0	NULL	executive functions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to controls , PD patients were impaired in all conditions and the severity of the deficit was significantly correlated with that observed in tests of executive functions .
	manualset3
247579	1	425447	7	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to the analysis of the X-ray results , 48 % of the one-track lethal damage caused by 5.1 MeV alpha particles ( approximately 88 keV/microm ) is due to intratrack DSB interactions while the remainder is due to other forms of one-track damage .
	manualset3
247580	2	425447	7	NULL	NULL	0	NULL	X-ray results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to the analysis of the X-ray results , 48 % of the one-track lethal damage caused by 5.1 MeV alpha particles ( approximately 88 keV/microm ) is due to intratrack DSB interactions while the remainder is due to other forms of one-track damage .
	manualset3
247581	3	425447	7	NULL	NULL	0	NULL	48 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to the analysis of the X-ray results , 48 % of the one-track lethal damage caused by 5.1 MeV alpha particles ( approximately 88 keV/microm ) is due to intratrack DSB interactions while the remainder is due to other forms of one-track damage .
	manualset3
247582	4	425447	7	NULL	NULL	0	NULL	one-track lethal damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to the analysis of the X-ray results , 48 % of the one-track lethal damage caused by 5.1 MeV alpha particles ( approximately 88 keV/microm ) is due to intratrack DSB interactions while the remainder is due to other forms of one-track damage .
	manualset3
247583	5	425447	7	NULL	NULL	0	NULL	5.1 MeV alpha particles	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to the analysis of the X-ray results , 48 % of the one-track lethal damage caused by 5.1 MeV alpha particles ( approximately 88 keV/microm ) is due to intratrack DSB interactions while the remainder is due to other forms of one-track damage .
	manualset3
247584	6	425447	7	NULL	NULL	0	NULL	88 keV/microm	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to the analysis of the X-ray results , 48 % of the one-track lethal damage caused by 5.1 MeV alpha particles ( approximately 88 keV/microm ) is due to intratrack DSB interactions while the remainder is due to other forms of one-track damage .
	manualset3
247585	7	425447	7	NULL	NULL	0	NULL	 intratrack DSB interactions 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to the analysis of the X-ray results , 48 % of the one-track lethal damage caused by 5.1 MeV alpha particles ( approximately 88 keV/microm ) is due to intratrack DSB interactions while the remainder is due to other forms of one-track damage .
	manualset3
247586	8	425447	7	NULL	NULL	0	NULL	remainder	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to the analysis of the X-ray results , 48 % of the one-track lethal damage caused by 5.1 MeV alpha particles ( approximately 88 keV/microm ) is due to intratrack DSB interactions while the remainder is due to other forms of one-track damage .
	manualset3
247587	9	425447	7	NULL	NULL	0	NULL	 forms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to the analysis of the X-ray results , 48 % of the one-track lethal damage caused by 5.1 MeV alpha particles ( approximately 88 keV/microm ) is due to intratrack DSB interactions while the remainder is due to other forms of one-track damage .
	manualset3
247588	10	425447	7	NULL	NULL	0	NULL	one-track damage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to the analysis of the X-ray results , 48 % of the one-track lethal damage caused by 5.1 MeV alpha particles ( approximately 88 keV/microm ) is due to intratrack DSB interactions while the remainder is due to other forms of one-track damage .
	manualset3
248052	1	425448	7	NULL	NULL	0	NULL	 Ionic influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Ionic influence on the structure of liposomal membranes , studied with the use of spon probes ) .
	manualset3
248053	2	425448	7	NULL	NULL	0	NULL	structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Ionic influence on the structure of liposomal membranes , studied with the use of spon probes ) .
	manualset3
248055	3	425448	7	NULL	NULL	0	NULL	liposomal membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	( Ionic influence on the structure of liposomal membranes , studied with the use of spon probes ) .
	manualset3
248056	4	425448	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Ionic influence on the structure of liposomal membranes , studied with the use of spon probes ) .
	manualset3
248058	5	425448	7	NULL	NULL	0	NULL	spon probes	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Ionic influence on the structure of liposomal membranes , studied with the use of spon probes ) .
	manualset3
248063	1	425449	7	NULL	NULL	0	NULL	control condition	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to the control condition with sham exposure , spectral power of the non-rapid eye movement sleep electroencephalogram ( EEG ) was initially increased in the 9-14 Hz range in both experiments .
	manualset3
248064	2	425449	7	NULL	NULL	0	NULL	sham exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to the control condition with sham exposure , spectral power of the non-rapid eye movement sleep electroencephalogram ( EEG ) was initially increased in the 9-14 Hz range in both experiments .
	manualset3
248086	3	425449	7	NULL	NULL	0	NULL	spectral power	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to the control condition with sham exposure , spectral power of the non-rapid eye movement sleep electroencephalogram ( EEG ) was initially increased in the 9-14 Hz range in both experiments .
	manualset3
248088	4	425449	7	NULL	NULL	0	NULL	 non-rapid eye movement sleep electroencephalogram ( EEG )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to the control condition with sham exposure , spectral power of the non-rapid eye movement sleep electroencephalogram ( EEG ) was initially increased in the 9-14 Hz range in both experiments .
	manualset3
248098	5	425449	7	NULL	NULL	0	NULL	9-14 Hz range 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to the control condition with sham exposure , spectral power of the non-rapid eye movement sleep electroencephalogram ( EEG ) was initially increased in the 9-14 Hz range in both experiments .
	manualset3
248099	6	425449	7	NULL	NULL	0	NULL	experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared to the control condition with sham exposure , spectral power of the non-rapid eye movement sleep electroencephalogram ( EEG ) was initially increased in the 9-14 Hz range in both experiments .
	manualset3
248112	1	425450	7	NULL	NULL	0	NULL	control levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with control levels , PI 4-K mRNA expression in the hippocampus , but not the cerebral cortex , was significantly decreased by 30 % and about 80 % 1 and 7 days after ischemia/reperfusion , respectively .
	manualset3
248113	2	425450	7	NULL	NULL	NULL	NULL	PI 4-K mRNA expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Compared with control levels , PI 4-K mRNA expression in the hippocampus , but not the cerebral cortex , was significantly decreased by 30 % and about 80 % 1 and 7 days after ischemia/reperfusion , respectively .
	manualset3
248114	3	425450	7	NULL	NULL	0	NULL	hippocampus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with control levels , PI 4-K mRNA expression in the hippocampus , but not the cerebral cortex , was significantly decreased by 30 % and about 80 % 1 and 7 days after ischemia/reperfusion , respectively .
	manualset3
248115	4	425450	7	NULL	NULL	0	NULL	cerebral cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with control levels , PI 4-K mRNA expression in the hippocampus , but not the cerebral cortex , was significantly decreased by 30 % and about 80 % 1 and 7 days after ischemia/reperfusion , respectively .
	manualset3
248116	5	425450	7	NULL	NULL	0	NULL	30 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with control levels , PI 4-K mRNA expression in the hippocampus , but not the cerebral cortex , was significantly decreased by 30 % and about 80 % 1 and 7 days after ischemia/reperfusion , respectively .
	manualset3
248117	6	425450	7	NULL	NULL	0	NULL	80 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with control levels , PI 4-K mRNA expression in the hippocampus , but not the cerebral cortex , was significantly decreased by 30 % and about 80 % 1 and 7 days after ischemia/reperfusion , respectively .
	manualset3
248118	7	425450	7	NULL	NULL	0	NULL	1 day	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with control levels , PI 4-K mRNA expression in the hippocampus , but not the cerebral cortex , was significantly decreased by 30 % and about 80 % 1 and 7 days after ischemia/reperfusion , respectively .
	manualset3
248119	8	425450	7	NULL	NULL	0	NULL	7 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with control levels , PI 4-K mRNA expression in the hippocampus , but not the cerebral cortex , was significantly decreased by 30 % and about 80 % 1 and 7 days after ischemia/reperfusion , respectively .
	manualset3
248120	9	425450	7	NULL	NULL	0	NULL	ischemia/reperfusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with control levels , PI 4-K mRNA expression in the hippocampus , but not the cerebral cortex , was significantly decreased by 30 % and about 80 % 1 and 7 days after ischemia/reperfusion , respectively .
	manualset3
248121	1	425451	7	NULL	NULL	0	NULL	 controls	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with controls , HZ cases had lower VZV-specific CD8 ( + ) CD107a ( + ) cell percentages independently of CD4 ( + ) percentages or HIV loads , suggesting that VZV-specific cytotoxic T cells are protective against HZ .
	manualset3
248122	2	425451	7	NULL	NULL	0	NULL	HZ cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with controls , HZ cases had lower VZV-specific CD8 ( + ) CD107a ( + ) cell percentages independently of CD4 ( + ) percentages or HIV loads , suggesting that VZV-specific cytotoxic T cells are protective against HZ .
	manualset3
248123	3	425451	7	NULL	NULL	0	NULL	lower VZV-specific CD8 ( + ) CD107a ( + ) cell percentages	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with controls , HZ cases had lower VZV-specific CD8 ( + ) CD107a ( + ) cell percentages independently of CD4 ( + ) percentages or HIV loads , suggesting that VZV-specific cytotoxic T cells are protective against HZ .
	manualset3
248124	4	425451	7	NULL	NULL	0	NULL	CD4 ( + ) percentages	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with controls , HZ cases had lower VZV-specific CD8 ( + ) CD107a ( + ) cell percentages independently of CD4 ( + ) percentages or HIV loads , suggesting that VZV-specific cytotoxic T cells are protective against HZ .
	manualset3
248125	5	425451	7	NULL	NULL	0	NULL	HIV loads	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with controls , HZ cases had lower VZV-specific CD8 ( + ) CD107a ( + ) cell percentages independently of CD4 ( + ) percentages or HIV loads , suggesting that VZV-specific cytotoxic T cells are protective against HZ .
	manualset3
248126	6	425451	7	NULL	NULL	0	NULL	VZV-specific cytotoxic T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with controls , HZ cases had lower VZV-specific CD8 ( + ) CD107a ( + ) cell percentages independently of CD4 ( + ) percentages or HIV loads , suggesting that VZV-specific cytotoxic T cells are protective against HZ .
	manualset3
248127	7	425451	7	NULL	NULL	0	NULL	HZ	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with controls , HZ cases had lower VZV-specific CD8 ( + ) CD107a ( + ) cell percentages independently of CD4 ( + ) percentages or HIV loads , suggesting that VZV-specific cytotoxic T cells are protective against HZ .
	manualset3
248128	1	425452	7	NULL	NULL	0	NULL	endocardial FS	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with endocardial FS , midwall FS had a stronger inverse association to LV mass ( r = -0.45 vs -0.16 , p & lt ; 0.001 ) .
	manualset3
248129	2	425452	7	NULL	NULL	0	NULL	midwall FS	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with endocardial FS , midwall FS had a stronger inverse association to LV mass ( r = -0.45 vs -0.16 , p & lt ; 0.001 ) .
	manualset3
248130	3	425452	7	NULL	NULL	0	NULL	inverse association	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with endocardial FS , midwall FS had a stronger inverse association to LV mass ( r = -0.45 vs -0.16 , p & lt ; 0.001 ) .
	manualset3
248131	4	425452	7	NULL	NULL	0	NULL	LV mass	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with endocardial FS , midwall FS had a stronger inverse association to LV mass ( r = -0.45 vs -0.16 , p & lt ; 0.001 ) .
	manualset3
248132	5	425452	7	NULL	NULL	0	NULL	r = -0.45	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with endocardial FS , midwall FS had a stronger inverse association to LV mass ( r = -0.45 vs -0.16 , p & lt ; 0.001 ) .
	manualset3
248133	6	425452	7	NULL	NULL	0	NULL	-0.16	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with endocardial FS , midwall FS had a stronger inverse association to LV mass ( r = -0.45 vs -0.16 , p & lt ; 0.001 ) .
	manualset3
248134	7	425452	7	NULL	NULL	0	NULL	p & lt ; 0.001	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with endocardial FS , midwall FS had a stronger inverse association to LV mass ( r = -0.45 vs -0.16 , p & lt ; 0.001 ) .
	manualset3
248135	1	425453	7	NULL	NULL	0	NULL	slow freezing methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with slow freezing methods , vitrification was less detrimental to cartilage cells and had a higher survival rate of chondrocytes and coverage of epithelium and cilia .
	manualset3
248136	2	425453	7	NULL	NULL	0	NULL	vitrification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with slow freezing methods , vitrification was less detrimental to cartilage cells and had a higher survival rate of chondrocytes and coverage of epithelium and cilia .
	manualset3
248137	3	425453	7	NULL	NULL	0	NULL	cartilage cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with slow freezing methods , vitrification was less detrimental to cartilage cells and had a higher survival rate of chondrocytes and coverage of epithelium and cilia .
	manualset3
248138	4	425453	7	NULL	NULL	0	NULL	higher survival rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with slow freezing methods , vitrification was less detrimental to cartilage cells and had a higher survival rate of chondrocytes and coverage of epithelium and cilia .
	manualset3
248139	5	425453	7	NULL	NULL	0	NULL	chondrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with slow freezing methods , vitrification was less detrimental to cartilage cells and had a higher survival rate of chondrocytes and coverage of epithelium and cilia .
	manualset3
248140	6	425453	7	NULL	NULL	0	NULL	coverage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with slow freezing methods , vitrification was less detrimental to cartilage cells and had a higher survival rate of chondrocytes and coverage of epithelium and cilia .
	manualset3
248141	7	425453	7	NULL	NULL	NULL	NULL	epithelium	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Compared with slow freezing methods , vitrification was less detrimental to cartilage cells and had a higher survival rate of chondrocytes and coverage of epithelium and cilia .
	manualset3
248142	8	425453	7	NULL	NULL	0	NULL	cilia	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with slow freezing methods , vitrification was less detrimental to cartilage cells and had a higher survival rate of chondrocytes and coverage of epithelium and cilia .
	manualset3
248143	1	425454	7	NULL	NULL	0	NULL	temporary deception	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with temporary deception , more attention resources were invested and intensely response conflict was induced by premeditated deception .
	manualset3
248144	2	425454	7	NULL	NULL	0	NULL	attention resources	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with temporary deception , more attention resources were invested and intensely response conflict was induced by premeditated deception .
	manualset3
248145	4	425454	7	NULL	NULL	NULL	NULL	premeditated deception 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Compared with temporary deception , more attention resources were invested and intensely response conflict was induced by premeditated deception .
	manualset3
248146	3	425454	7	NULL	NULL	0	NULL	intensely response conflict	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with temporary deception , more attention resources were invested and intensely response conflict was induced by premeditated deception .
	manualset3
248147	1	425455	7	NULL	NULL	0	NULL	 CV values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the CV values obtained from the commercial machine in the range of 4.33-14 .56 % , it is noted that CV values of the prototype with respect to the samples of different initial concentration ranging from 10 ( 7 ) to 10 ( 3 ) copies/ml are almost equable .
	manualset3
248148	2	425455	7	NULL	NULL	0	NULL	 commercial machine	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the CV values obtained from the commercial machine in the range of 4.33-14 .56 % , it is noted that CV values of the prototype with respect to the samples of different initial concentration ranging from 10 ( 7 ) to 10 ( 3 ) copies/ml are almost equable .
	manualset3
248149	3	425455	7	NULL	NULL	0	NULL	 range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the CV values obtained from the commercial machine in the range of 4.33-14 .56 % , it is noted that CV values of the prototype with respect to the samples of different initial concentration ranging from 10 ( 7 ) to 10 ( 3 ) copies/ml are almost equable .
	manualset3
248150	4	425455	7	NULL	NULL	0	NULL	4.33-14 .56 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the CV values obtained from the commercial machine in the range of 4.33-14 .56 % , it is noted that CV values of the prototype with respect to the samples of different initial concentration ranging from 10 ( 7 ) to 10 ( 3 ) copies/ml are almost equable .
	manualset3
248151	5	425455	7	NULL	NULL	0	NULL	CV values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the CV values obtained from the commercial machine in the range of 4.33-14 .56 % , it is noted that CV values of the prototype with respect to the samples of different initial concentration ranging from 10 ( 7 ) to 10 ( 3 ) copies/ml are almost equable .
	manualset3
248152	6	425455	7	NULL	NULL	0	NULL	 prototype	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the CV values obtained from the commercial machine in the range of 4.33-14 .56 % , it is noted that CV values of the prototype with respect to the samples of different initial concentration ranging from 10 ( 7 ) to 10 ( 3 ) copies/ml are almost equable .
	manualset3
248153	7	425455	7	NULL	NULL	0	NULL	samples	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the CV values obtained from the commercial machine in the range of 4.33-14 .56 % , it is noted that CV values of the prototype with respect to the samples of different initial concentration ranging from 10 ( 7 ) to 10 ( 3 ) copies/ml are almost equable .
	manualset3
248154	8	425455	7	NULL	NULL	0	NULL	different initial concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the CV values obtained from the commercial machine in the range of 4.33-14 .56 % , it is noted that CV values of the prototype with respect to the samples of different initial concentration ranging from 10 ( 7 ) to 10 ( 3 ) copies/ml are almost equable .
	manualset3
248155	9	425455	7	NULL	NULL	0	NULL	10 ( 7 ) copies/ml	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the CV values obtained from the commercial machine in the range of 4.33-14 .56 % , it is noted that CV values of the prototype with respect to the samples of different initial concentration ranging from 10 ( 7 ) to 10 ( 3 ) copies/ml are almost equable .
	manualset3
248156	10	425455	7	NULL	NULL	0	NULL	10 ( 3 ) copies/ml	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the CV values obtained from the commercial machine in the range of 4.33-14 .56 % , it is noted that CV values of the prototype with respect to the samples of different initial concentration ranging from 10 ( 7 ) to 10 ( 3 ) copies/ml are almost equable .
	manualset3
248157	1	425456	7	NULL	NULL	0	NULL	main vessel	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the main vessel , side branch lesions were shorter , with a smaller reference diameter and final in-stent minimum lumen diameter .
	manualset3
248158	2	425456	7	NULL	NULL	0	NULL	side branch lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the main vessel , side branch lesions were shorter , with a smaller reference diameter and final in-stent minimum lumen diameter .
	manualset3
248159	3	425456	7	NULL	NULL	0	NULL	smaller reference diameter 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the main vessel , side branch lesions were shorter , with a smaller reference diameter and final in-stent minimum lumen diameter .
	manualset3
248160	4	425456	7	NULL	NULL	NULL	NULL	final in-stent minimum lumen diameter	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Compared with the main vessel , side branch lesions were shorter , with a smaller reference diameter and final in-stent minimum lumen diameter .
	manualset3
248163	1	425457	7	NULL	NULL	0	NULL	Irradiation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Irradiation of the epipharynx with radiocobalt in sound conduction disorders ) .
	manualset3
248164	2	425457	7	NULL	NULL	0	NULL	 epipharynx	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Irradiation of the epipharynx with radiocobalt in sound conduction disorders ) .
	manualset3
248165	3	425457	7	NULL	NULL	0	NULL	radiocobalt	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Irradiation of the epipharynx with radiocobalt in sound conduction disorders ) .
	manualset3
248167	4	425457	7	NULL	NULL	0	NULL	sound conduction disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Irradiation of the epipharynx with radiocobalt in sound conduction disorders ) .
	manualset3
248168	1	425458	7	NULL	NULL	0	NULL	original clay	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the original clay , copper loaded samples showed new DTGA peaks assigned to NH ( 3 ) and N ( 2 ) O. The presence of the N ( 2 ) O peak suggested that the loaded copper species were in agglomerated copper oxide form , which dispersed well over the edges and external surfaces of the clay layers .
	manualset3
248170	2	425458	7	NULL	NULL	0	NULL	copper loaded samples	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the original clay , copper loaded samples showed new DTGA peaks assigned to NH ( 3 ) and N ( 2 ) O. The presence of the N ( 2 ) O peak suggested that the loaded copper species were in agglomerated copper oxide form , which dispersed well over the edges and external surfaces of the clay layers .
	manualset3
248171	3	425458	7	NULL	NULL	0	NULL	new DTGA peaks	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the original clay , copper loaded samples showed new DTGA peaks assigned to NH ( 3 ) and N ( 2 ) O. The presence of the N ( 2 ) O peak suggested that the loaded copper species were in agglomerated copper oxide form , which dispersed well over the edges and external surfaces of the clay layers .
	manualset3
248172	4	425458	7	NULL	NULL	0	NULL	NH ( 3 ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the original clay , copper loaded samples showed new DTGA peaks assigned to NH ( 3 ) and N ( 2 ) O. The presence of the N ( 2 ) O peak suggested that the loaded copper species were in agglomerated copper oxide form , which dispersed well over the edges and external surfaces of the clay layers .
	manualset3
248173	5	425458	7	NULL	NULL	0	NULL	N ( 2 ) O	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the original clay , copper loaded samples showed new DTGA peaks assigned to NH ( 3 ) and N ( 2 ) O. The presence of the N ( 2 ) O peak suggested that the loaded copper species were in agglomerated copper oxide form , which dispersed well over the edges and external surfaces of the clay layers .
	manualset3
248174	6	425458	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the original clay , copper loaded samples showed new DTGA peaks assigned to NH ( 3 ) and N ( 2 ) O. The presence of the N ( 2 ) O peak suggested that the loaded copper species were in agglomerated copper oxide form , which dispersed well over the edges and external surfaces of the clay layers .
	manualset3
248176	7	425458	7	NULL	NULL	0	NULL	N ( 2 ) O peak 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the original clay , copper loaded samples showed new DTGA peaks assigned to NH ( 3 ) and N ( 2 ) O. The presence of the N ( 2 ) O peak suggested that the loaded copper species were in agglomerated copper oxide form , which dispersed well over the edges and external surfaces of the clay layers .
	manualset3
248177	8	425458	7	NULL	NULL	0	NULL	loaded copper species	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the original clay , copper loaded samples showed new DTGA peaks assigned to NH ( 3 ) and N ( 2 ) O. The presence of the N ( 2 ) O peak suggested that the loaded copper species were in agglomerated copper oxide form , which dispersed well over the edges and external surfaces of the clay layers .
	manualset3
248178	9	425458	7	NULL	NULL	0	NULL	agglomerated copper oxide form	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the original clay , copper loaded samples showed new DTGA peaks assigned to NH ( 3 ) and N ( 2 ) O. The presence of the N ( 2 ) O peak suggested that the loaded copper species were in agglomerated copper oxide form , which dispersed well over the edges and external surfaces of the clay layers .
	manualset3
248179	10	425458	7	NULL	NULL	0	NULL	edges	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the original clay , copper loaded samples showed new DTGA peaks assigned to NH ( 3 ) and N ( 2 ) O. The presence of the N ( 2 ) O peak suggested that the loaded copper species were in agglomerated copper oxide form , which dispersed well over the edges and external surfaces of the clay layers .
	manualset3
248180	11	425458	7	NULL	NULL	0	NULL	external surfaces	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the original clay , copper loaded samples showed new DTGA peaks assigned to NH ( 3 ) and N ( 2 ) O. The presence of the N ( 2 ) O peak suggested that the loaded copper species were in agglomerated copper oxide form , which dispersed well over the edges and external surfaces of the clay layers .
	manualset3
248181	12	425458	7	NULL	NULL	0	NULL	clay layers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the original clay , copper loaded samples showed new DTGA peaks assigned to NH ( 3 ) and N ( 2 ) O. The presence of the N ( 2 ) O peak suggested that the loaded copper species were in agglomerated copper oxide form , which dispersed well over the edges and external surfaces of the clay layers .
	manualset3
248182	1	425459	7	NULL	NULL	0	NULL	 solvent control group 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the solvent control group ( trioctanoin ) , both NNN and NNK induced significant numbers of tumors of the nasal cavity ( P less than 0.01 ) at all three dose levels in both male and female rats .
	manualset3
248183	2	425459	7	NULL	NULL	0	NULL	trioctanoin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the solvent control group ( trioctanoin ) , both NNN and NNK induced significant numbers of tumors of the nasal cavity ( P less than 0.01 ) at all three dose levels in both male and female rats .
	manualset3
248184	3	425459	7	NULL	NULL	0	NULL	NNN	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the solvent control group ( trioctanoin ) , both NNN and NNK induced significant numbers of tumors of the nasal cavity ( P less than 0.01 ) at all three dose levels in both male and female rats .
	manualset3
248185	4	425459	7	NULL	NULL	0	NULL	NNK 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the solvent control group ( trioctanoin ) , both NNN and NNK induced significant numbers of tumors of the nasal cavity ( P less than 0.01 ) at all three dose levels in both male and female rats .
	manualset3
248186	5	425459	7	NULL	NULL	0	NULL	numbers	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the solvent control group ( trioctanoin ) , both NNN and NNK induced significant numbers of tumors of the nasal cavity ( P less than 0.01 ) at all three dose levels in both male and female rats .
	manualset3
248187	6	425459	7	NULL	NULL	0	NULL	 tumors 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the solvent control group ( trioctanoin ) , both NNN and NNK induced significant numbers of tumors of the nasal cavity ( P less than 0.01 ) at all three dose levels in both male and female rats .
	manualset3
248188	7	425459	7	NULL	NULL	0	NULL	nasal cavity	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the solvent control group ( trioctanoin ) , both NNN and NNK induced significant numbers of tumors of the nasal cavity ( P less than 0.01 ) at all three dose levels in both male and female rats .
	manualset3
248189	8	425459	7	NULL	NULL	0	NULL	P less than 0.01	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the solvent control group ( trioctanoin ) , both NNN and NNK induced significant numbers of tumors of the nasal cavity ( P less than 0.01 ) at all three dose levels in both male and female rats .
	manualset3
248190	9	425459	7	NULL	NULL	0	NULL	three dose levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the solvent control group ( trioctanoin ) , both NNN and NNK induced significant numbers of tumors of the nasal cavity ( P less than 0.01 ) at all three dose levels in both male and female rats .
	manualset3
248191	10	425459	7	NULL	NULL	0	NULL	male rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the solvent control group ( trioctanoin ) , both NNN and NNK induced significant numbers of tumors of the nasal cavity ( P less than 0.01 ) at all three dose levels in both male and female rats .
	manualset3
248192	11	425459	7	NULL	NULL	0	NULL	female rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Compared with the solvent control group ( trioctanoin ) , both NNN and NNK induced significant numbers of tumors of the nasal cavity ( P less than 0.01 ) at all three dose levels in both male and female rats .
	manualset3
248193	1	425460	7	NULL	NULL	0	NULL	dissolution rates	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the dissolution rates of terpene lactones and flavone glycosides within the single products , most were approximately the same .
	manualset3
248194	2	425460	7	NULL	NULL	0	NULL	terpene lactones 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the dissolution rates of terpene lactones and flavone glycosides within the single products , most were approximately the same .
	manualset3
248195	3	425460	7	NULL	NULL	0	NULL	flavone glycosides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the dissolution rates of terpene lactones and flavone glycosides within the single products , most were approximately the same .
	manualset3
248196	4	425460	7	NULL	NULL	0	NULL	single products	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the dissolution rates of terpene lactones and flavone glycosides within the single products , most were approximately the same .
	manualset3
248197	5	425460	7	NULL	NULL	0	NULL	comparing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the dissolution rates of terpene lactones and flavone glycosides within the single products , most were approximately the same .
	manualset3
248717	1	425461	7	NULL	NULL	0	NULL	Comparing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the effectiveness of the mini-lecture technique to role-playing in a dental psychology course .
	manualset3
248718	2	425461	7	NULL	NULL	0	NULL	 effectiveness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the effectiveness of the mini-lecture technique to role-playing in a dental psychology course .
	manualset3
248719	3	425461	7	NULL	NULL	0	NULL	mini-lecture technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the effectiveness of the mini-lecture technique to role-playing in a dental psychology course .
	manualset3
248721	4	425461	7	NULL	NULL	0	NULL	dental psychology course	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the effectiveness of the mini-lecture technique to role-playing in a dental psychology course .
	manualset3
248726	1	425462	7	NULL	NULL	0	NULL	Comparing 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the structure with published data of similar compounds shows that the Ge-O bonds are covalent and the Ge-N bond is coordinated .
	manualset3
248727	2	425462	7	NULL	NULL	0	NULL	structure 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the structure with published data of similar compounds shows that the Ge-O bonds are covalent and the Ge-N bond is coordinated .
	manualset3
248729	3	425462	7	NULL	NULL	0	NULL	 published data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the structure with published data of similar compounds shows that the Ge-O bonds are covalent and the Ge-N bond is coordinated .
	manualset3
248731	4	425462	7	NULL	NULL	0	NULL	compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the structure with published data of similar compounds shows that the Ge-O bonds are covalent and the Ge-N bond is coordinated .
	manualset3
248732	5	425462	7	NULL	NULL	0	NULL	Ge-O bonds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the structure with published data of similar compounds shows that the Ge-O bonds are covalent and the Ge-N bond is coordinated .
	manualset3
248733	6	425462	7	NULL	NULL	0	NULL	Ge-N bond	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the structure with published data of similar compounds shows that the Ge-O bonds are covalent and the Ge-N bond is coordinated .
	manualset3
248736	1	425463	7	NULL	NULL	0	NULL	Comparing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the synthetic response of fibroblasts obtained from young and old donors , we observed a marked increase of the inhibition of type I and type VI collagen expression and the stimulation of interstitial collagenase in the aged fibroblasts .
	manualset3
248738	2	425463	7	NULL	NULL	0	NULL	synthetic response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the synthetic response of fibroblasts obtained from young and old donors , we observed a marked increase of the inhibition of type I and type VI collagen expression and the stimulation of interstitial collagenase in the aged fibroblasts .
	manualset3
248740	3	425463	7	NULL	NULL	0	NULL	fibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the synthetic response of fibroblasts obtained from young and old donors , we observed a marked increase of the inhibition of type I and type VI collagen expression and the stimulation of interstitial collagenase in the aged fibroblasts .
	manualset3
248742	4	425463	7	NULL	NULL	0	NULL	young donors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the synthetic response of fibroblasts obtained from young and old donors , we observed a marked increase of the inhibition of type I and type VI collagen expression and the stimulation of interstitial collagenase in the aged fibroblasts .
	manualset3
248743	5	425463	7	NULL	NULL	0	NULL	old donors	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the synthetic response of fibroblasts obtained from young and old donors , we observed a marked increase of the inhibition of type I and type VI collagen expression and the stimulation of interstitial collagenase in the aged fibroblasts .
	manualset3
248744	6	425463	7	NULL	NULL	NULL	NULL	marked increase	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Comparing the synthetic response of fibroblasts obtained from young and old donors , we observed a marked increase of the inhibition of type I and type VI collagen expression and the stimulation of interstitial collagenase in the aged fibroblasts .
	manualset3
248745	7	425463	7	NULL	NULL	0	NULL	 inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the synthetic response of fibroblasts obtained from young and old donors , we observed a marked increase of the inhibition of type I and type VI collagen expression and the stimulation of interstitial collagenase in the aged fibroblasts .
	manualset3
248746	8	425463	7	NULL	NULL	0	NULL	type I collagen expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the synthetic response of fibroblasts obtained from young and old donors , we observed a marked increase of the inhibition of type I and type VI collagen expression and the stimulation of interstitial collagenase in the aged fibroblasts .
	manualset3
248747	9	425463	7	NULL	NULL	0	NULL	stimulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the synthetic response of fibroblasts obtained from young and old donors , we observed a marked increase of the inhibition of type I and type VI collagen expression and the stimulation of interstitial collagenase in the aged fibroblasts .
	manualset3
248748	10	425463	7	NULL	NULL	0	NULL	 interstitial collagenase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the synthetic response of fibroblasts obtained from young and old donors , we observed a marked increase of the inhibition of type I and type VI collagen expression and the stimulation of interstitial collagenase in the aged fibroblasts .
	manualset3
248749	11	425463	7	NULL	NULL	0	NULL	aged fibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the synthetic response of fibroblasts obtained from young and old donors , we observed a marked increase of the inhibition of type I and type VI collagen expression and the stimulation of interstitial collagenase in the aged fibroblasts .
	manualset3
248751	12	425463	7	NULL	NULL	0	NULL	 type VI collagen expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparing the synthetic response of fibroblasts obtained from young and old donors , we observed a marked increase of the inhibition of type I and type VI collagen expression and the stimulation of interstitial collagenase in the aged fibroblasts .
	manualset3
248753	1	425464	7	NULL	NULL	0	NULL	Comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison between insulin-like growth factor-I ( IGF-I ) and IGF binding protein-3 ( IGFBP-3 ) measurement in the diagnosis of growth hormone deficiency .
	manualset3
248754	2	425464	7	NULL	NULL	0	NULL	insulin-like growth factor-I ( IGF-I ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison between insulin-like growth factor-I ( IGF-I ) and IGF binding protein-3 ( IGFBP-3 ) measurement in the diagnosis of growth hormone deficiency .
	manualset3
248755	3	425464	7	NULL	NULL	0	NULL	IGF binding protein-3 ( IGFBP-3 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison between insulin-like growth factor-I ( IGF-I ) and IGF binding protein-3 ( IGFBP-3 ) measurement in the diagnosis of growth hormone deficiency .
	manualset3
248757	4	425464	7	NULL	NULL	0	NULL	measurement	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison between insulin-like growth factor-I ( IGF-I ) and IGF binding protein-3 ( IGFBP-3 ) measurement in the diagnosis of growth hormone deficiency .
	manualset3
248758	5	425464	7	NULL	NULL	0	NULL	diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison between insulin-like growth factor-I ( IGF-I ) and IGF binding protein-3 ( IGFBP-3 ) measurement in the diagnosis of growth hormone deficiency .
	manualset3
248759	6	425464	7	NULL	NULL	0	NULL	growth hormone deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison between insulin-like growth factor-I ( IGF-I ) and IGF binding protein-3 ( IGFBP-3 ) measurement in the diagnosis of growth hormone deficiency .
	manualset3
248760	1	425465	7	NULL	NULL	0	NULL	Comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of Bifidobacterium breve strain Yakult transcriptomes in germ-free mice with those in fecal cultures .
	manualset3
248761	2	425465	7	NULL	NULL	0	NULL	Bifidobacterium breve strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of Bifidobacterium breve strain Yakult transcriptomes in germ-free mice with those in fecal cultures .
	manualset3
248762	3	425465	7	NULL	NULL	0	NULL	Yakult transcriptomes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of Bifidobacterium breve strain Yakult transcriptomes in germ-free mice with those in fecal cultures .
	manualset3
248763	4	425465	7	NULL	NULL	0	NULL	germ-free mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of Bifidobacterium breve strain Yakult transcriptomes in germ-free mice with those in fecal cultures .
	manualset3
248764	5	425465	7	NULL	NULL	0	NULL	fecal cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of Bifidobacterium breve strain Yakult transcriptomes in germ-free mice with those in fecal cultures .
	manualset3
248765	1	425466	7	NULL	NULL	0	NULL	benign breast disease 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Is benign breast disease a contra-indication to hormone replacement therapy ? ) .
	manualset3
248766	2	425466	7	NULL	NULL	0	NULL	contra-indication 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Is benign breast disease a contra-indication to hormone replacement therapy ? ) .
	manualset3
248767	3	425466	7	NULL	NULL	0	NULL	hormone replacement therapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Is benign breast disease a contra-indication to hormone replacement therapy ? ) .
	manualset3
248824	1	425467	7	NULL	NULL	0	NULL	Comparison 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of CI and THICI showed no statistically significant differences for any of the parameters studied .
	manualset3
248825	2	425467	7	NULL	NULL	0	NULL	CI	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of CI and THICI showed no statistically significant differences for any of the parameters studied .
	manualset3
248826	3	425467	7	NULL	NULL	0	NULL	THICI	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of CI and THICI showed no statistically significant differences for any of the parameters studied .
	manualset3
248827	4	425467	7	NULL	NULL	0	NULL	statistically significant differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of CI and THICI showed no statistically significant differences for any of the parameters studied .
	manualset3
248828	5	425467	7	NULL	NULL	0	NULL	parameters	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of CI and THICI showed no statistically significant differences for any of the parameters studied .
	manualset3
248829	1	425468	7	NULL	NULL	0	NULL	Comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of CMT1A and CMT2 : similarities and differences .
	manualset3
248830	2	425468	7	NULL	NULL	0	NULL	CMT1A	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of CMT1A and CMT2 : similarities and differences .
	manualset3
248831	3	425468	7	NULL	NULL	0	NULL	CMT2	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of CMT1A and CMT2 : similarities and differences .
	manualset3
251147	4	425468	7	NULL	NULL	0	NULL	 similarities 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of CMT1A and CMT2 : similarities and differences .
	manualset3
251148	5	425468	7	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of CMT1A and CMT2 : similarities and differences .
	manualset3
248832	1	425469	7	NULL	NULL	0	NULL	Comparison 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of QT dispersion during atrial fibrillation and sinus rhythm in the same patients , at normal and prolonged ventricular repolarization .
	manualset3
248833	2	425469	7	NULL	NULL	0	NULL	QT dispersion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of QT dispersion during atrial fibrillation and sinus rhythm in the same patients , at normal and prolonged ventricular repolarization .
	manualset3
248841	3	425469	7	NULL	NULL	0	NULL	atrial fibrillation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of QT dispersion during atrial fibrillation and sinus rhythm in the same patients , at normal and prolonged ventricular repolarization .
	manualset3
248842	4	425469	7	NULL	NULL	0	NULL	sinus rhythm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of QT dispersion during atrial fibrillation and sinus rhythm in the same patients , at normal and prolonged ventricular repolarization .
	manualset3
248843	5	425469	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of QT dispersion during atrial fibrillation and sinus rhythm in the same patients , at normal and prolonged ventricular repolarization .
	manualset3
248844	6	425469	7	NULL	NULL	0	NULL	 normal repolarization 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of QT dispersion during atrial fibrillation and sinus rhythm in the same patients , at normal and prolonged ventricular repolarization .
	manualset3
248845	7	425469	7	NULL	NULL	0	NULL	 prolonged ventricular repolarization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of QT dispersion during atrial fibrillation and sinus rhythm in the same patients , at normal and prolonged ventricular repolarization .
	manualset3
248846	1	425470	7	NULL	NULL	0	NULL	Comparison 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of acetaminophen and ketoprofen in febrile children : a single dose randomized clinical trial .
	manualset3
248847	2	425470	7	NULL	NULL	0	NULL	acetaminophen 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of acetaminophen and ketoprofen in febrile children : a single dose randomized clinical trial .
	manualset3
248848	3	425470	7	NULL	NULL	0	NULL	 ketoprofen	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of acetaminophen and ketoprofen in febrile children : a single dose randomized clinical trial .
	manualset3
248849	4	425470	7	NULL	NULL	0	NULL	febrile children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of acetaminophen and ketoprofen in febrile children : a single dose randomized clinical trial .
	manualset3
248850	5	425470	7	NULL	NULL	0	NULL	single dose randomized clinical trial	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of acetaminophen and ketoprofen in febrile children : a single dose randomized clinical trial .
	manualset3
248851	1	425471	7	NULL	NULL	0	NULL	Comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of airway management with the intubating laryngeal mask , laryngeal tube and CobraPLA by paramedical students in anaesthetized patients .
	manualset3
248852	2	425471	7	NULL	NULL	0	NULL	airway management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of airway management with the intubating laryngeal mask , laryngeal tube and CobraPLA by paramedical students in anaesthetized patients .
	manualset3
248853	3	425471	7	NULL	NULL	0	NULL	laryngeal mask	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of airway management with the intubating laryngeal mask , laryngeal tube and CobraPLA by paramedical students in anaesthetized patients .
	manualset3
248854	4	425471	7	NULL	NULL	0	NULL	 laryngeal tube	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of airway management with the intubating laryngeal mask , laryngeal tube and CobraPLA by paramedical students in anaesthetized patients .
	manualset3
248855	5	425471	7	NULL	NULL	0	NULL	CobraPLA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of airway management with the intubating laryngeal mask , laryngeal tube and CobraPLA by paramedical students in anaesthetized patients .
	manualset3
248856	6	425471	7	NULL	NULL	0	NULL	paramedical students	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of airway management with the intubating laryngeal mask , laryngeal tube and CobraPLA by paramedical students in anaesthetized patients .
	manualset3
248857	7	425471	7	NULL	NULL	0	NULL	anaesthetized patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of airway management with the intubating laryngeal mask , laryngeal tube and CobraPLA by paramedical students in anaesthetized patients .
	manualset3
248858	1	425472	7	NULL	NULL	0	NULL	Comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of antinicotinic activity by neosurugatoxin and the structurally related compounds .
	manualset3
248859	2	425472	7	NULL	NULL	0	NULL	antinicotinic activity 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of antinicotinic activity by neosurugatoxin and the structurally related compounds .
	manualset3
248860	3	425472	7	NULL	NULL	0	NULL	neosurugatoxin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of antinicotinic activity by neosurugatoxin and the structurally related compounds .
	manualset3
248862	4	425472	7	NULL	NULL	0	NULL	related compounds	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of antinicotinic activity by neosurugatoxin and the structurally related compounds .
	manualset3
248864	1	425473	7	NULL	NULL	0	NULL	Comparison 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of buccal nitroglycerin and oral isosorbide dinitrate for nitrate tolerance in stable angina pectoris .
	manualset3
248865	2	425473	7	NULL	NULL	0	NULL	buccal nitroglycerin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of buccal nitroglycerin and oral isosorbide dinitrate for nitrate tolerance in stable angina pectoris .
	manualset3
248866	3	425473	7	NULL	NULL	0	NULL	oral isosorbide dinitrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of buccal nitroglycerin and oral isosorbide dinitrate for nitrate tolerance in stable angina pectoris .
	manualset3
248868	4	425473	7	NULL	NULL	0	NULL	nitrate tolerance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of buccal nitroglycerin and oral isosorbide dinitrate for nitrate tolerance in stable angina pectoris .
	manualset3
248869	5	425473	7	NULL	NULL	0	NULL	stable angina pectoris	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of buccal nitroglycerin and oral isosorbide dinitrate for nitrate tolerance in stable angina pectoris .
	manualset3
248871	1	425474	7	NULL	NULL	0	NULL	Comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of different uncertainty techniques in urban stormwater quantity and quality modelling .
	manualset3
248872	2	425474	7	NULL	NULL	0	NULL	uncertainty techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of different uncertainty techniques in urban stormwater quantity and quality modelling .
	manualset3
248874	3	425474	7	NULL	NULL	0	NULL	urban stormwater quantity modelling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of different uncertainty techniques in urban stormwater quantity and quality modelling .
	manualset3
248875	4	425474	7	NULL	NULL	0	NULL	quality modelling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of different uncertainty techniques in urban stormwater quantity and quality modelling .
	manualset3
248876	1	425475	7	NULL	NULL	0	NULL	Comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of fluorescence quantum yields , excited state lifetimes and absorption characteristics indicate similar light-harvesting properties of the DV-Chls as their monovinyl counterparts .
	manualset3
248877	2	425475	7	NULL	NULL	0	NULL	fluorescence quantum yields	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of fluorescence quantum yields , excited state lifetimes and absorption characteristics indicate similar light-harvesting properties of the DV-Chls as their monovinyl counterparts .
	manualset3
248878	3	425475	7	NULL	NULL	NULL	NULL	 excited state lifetimes 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Comparison of fluorescence quantum yields , excited state lifetimes and absorption characteristics indicate similar light-harvesting properties of the DV-Chls as their monovinyl counterparts .
	manualset3
248879	4	425475	7	NULL	NULL	0	NULL	absorption characteristics	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of fluorescence quantum yields , excited state lifetimes and absorption characteristics indicate similar light-harvesting properties of the DV-Chls as their monovinyl counterparts .
	manualset3
248880	5	425475	7	NULL	NULL	0	NULL	light-harvesting properties	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of fluorescence quantum yields , excited state lifetimes and absorption characteristics indicate similar light-harvesting properties of the DV-Chls as their monovinyl counterparts .
	manualset3
248882	6	425475	7	NULL	NULL	0	NULL	DV-Chls	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of fluorescence quantum yields , excited state lifetimes and absorption characteristics indicate similar light-harvesting properties of the DV-Chls as their monovinyl counterparts .
	manualset3
248883	7	425475	7	NULL	NULL	0	NULL	monovinyl counterparts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of fluorescence quantum yields , excited state lifetimes and absorption characteristics indicate similar light-harvesting properties of the DV-Chls as their monovinyl counterparts .
	manualset3
248885	1	425476	7	NULL	NULL	0	NULL	Comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of gastritis and gastric epithelial proliferation in Helicobacter heilmannii-infected nude and BALB/c mice .
	manualset3
248886	2	425476	7	NULL	NULL	0	NULL	gastritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of gastritis and gastric epithelial proliferation in Helicobacter heilmannii-infected nude and BALB/c mice .
	manualset3
248888	3	425476	7	NULL	NULL	0	NULL	gastric epithelial proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of gastritis and gastric epithelial proliferation in Helicobacter heilmannii-infected nude and BALB/c mice .
	manualset3
248889	4	425476	7	NULL	NULL	0	NULL	Helicobacter heilmannii-infected nude mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of gastritis and gastric epithelial proliferation in Helicobacter heilmannii-infected nude and BALB/c mice .
	manualset3
248890	5	425476	7	NULL	NULL	0	NULL	BALB/c mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of gastritis and gastric epithelial proliferation in Helicobacter heilmannii-infected nude and BALB/c mice .
	manualset3
248891	1	425477	7	NULL	NULL	0	NULL	Comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of head circumference in an Israeli child population with United States and British standards .
	manualset3
248892	2	425477	7	NULL	NULL	0	NULL	head circumference	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of head circumference in an Israeli child population with United States and British standards .
	manualset3
248893	3	425477	7	NULL	NULL	0	NULL	Israeli child population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of head circumference in an Israeli child population with United States and British standards .
	manualset3
248894	4	425477	7	NULL	NULL	0	NULL	United States 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of head circumference in an Israeli child population with United States and British standards .
	manualset3
248895	5	425477	7	NULL	NULL	NULL	NULL	British standards 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Comparison of head circumference in an Israeli child population with United States and British standards .
	manualset3
248896	1	425478	7	NULL	NULL	0	NULL	Comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of ligand-induced conformational changes and domain closure mechanisms , between prokaryotic and eukaryotic dehydroquinate synthases .
	manualset3
248897	2	425478	7	NULL	NULL	0	NULL	ligand-induced conformational changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of ligand-induced conformational changes and domain closure mechanisms , between prokaryotic and eukaryotic dehydroquinate synthases .
	manualset3
248898	3	425478	7	NULL	NULL	0	NULL	domain closure mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of ligand-induced conformational changes and domain closure mechanisms , between prokaryotic and eukaryotic dehydroquinate synthases .
	manualset3
248899	4	425478	7	NULL	NULL	0	NULL	prokaryotic dehydroquinate synthases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of ligand-induced conformational changes and domain closure mechanisms , between prokaryotic and eukaryotic dehydroquinate synthases .
	manualset3
248900	5	425478	7	NULL	NULL	0	NULL	eukaryotic dehydroquinate synthases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of ligand-induced conformational changes and domain closure mechanisms , between prokaryotic and eukaryotic dehydroquinate synthases .
	manualset3
248901	1	425479	7	NULL	NULL	0	NULL	Comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of low-dose dobutamine-gradient-echo magnetic resonance imaging and positron emission tomography with ( 18F ) fluorodeoxyglucose in patients with chronic coronary artery disease .
	manualset3
248902	2	425479	7	NULL	NULL	0	NULL	 low-dose dobutamine-gradient-echo magnetic resonance imaging	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of low-dose dobutamine-gradient-echo magnetic resonance imaging and positron emission tomography with ( 18F ) fluorodeoxyglucose in patients with chronic coronary artery disease .
	manualset3
248903	3	425479	7	NULL	NULL	0	NULL	 positron emission tomography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of low-dose dobutamine-gradient-echo magnetic resonance imaging and positron emission tomography with ( 18F ) fluorodeoxyglucose in patients with chronic coronary artery disease .
	manualset3
248904	4	425479	7	NULL	NULL	0	NULL	( 18F ) fluorodeoxyglucose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of low-dose dobutamine-gradient-echo magnetic resonance imaging and positron emission tomography with ( 18F ) fluorodeoxyglucose in patients with chronic coronary artery disease .
	manualset3
248906	5	425479	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of low-dose dobutamine-gradient-echo magnetic resonance imaging and positron emission tomography with ( 18F ) fluorodeoxyglucose in patients with chronic coronary artery disease .
	manualset3
248907	6	425479	7	NULL	NULL	0	NULL	chronic coronary artery disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of low-dose dobutamine-gradient-echo magnetic resonance imaging and positron emission tomography with ( 18F ) fluorodeoxyglucose in patients with chronic coronary artery disease .
	manualset3
248908	1	425480	7	NULL	NULL	0	NULL	Comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of oxidative damage in Malaysian end-stage renal disease patients with or without non-insulin-dependent diabetes mellitus .
	manualset3
248909	2	425480	7	NULL	NULL	0	NULL	oxidative damage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of oxidative damage in Malaysian end-stage renal disease patients with or without non-insulin-dependent diabetes mellitus .
	manualset3
248910	3	425480	7	NULL	NULL	0	NULL	Malaysian end-stage renal disease patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of oxidative damage in Malaysian end-stage renal disease patients with or without non-insulin-dependent diabetes mellitus .
	manualset3
248911	4	425480	7	NULL	NULL	0	NULL	non-insulin-dependent diabetes mellitus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of oxidative damage in Malaysian end-stage renal disease patients with or without non-insulin-dependent diabetes mellitus .
	manualset3
248945	1	425481	7	NULL	NULL	0	NULL	Comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of pediatric Clarion recipients with and without the electrode positioner .
	manualset3
248946	2	425481	7	NULL	NULL	0	NULL	pediatric Clarion recipients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of pediatric Clarion recipients with and without the electrode positioner .
	manualset3
248947	3	425481	7	NULL	NULL	0	NULL	electrode positioner	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of pediatric Clarion recipients with and without the electrode positioner .
	manualset3
248948	1	425482	7	NULL	NULL	0	NULL	migraine	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Is migraine a neuronal channelopothy ? ) .
	manualset3
248949	2	425482	7	NULL	NULL	0	NULL	neuronal channelopothy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Is migraine a neuronal channelopothy ? ) .
	manualset3
248950	1	425483	7	NULL	NULL	0	NULL	Comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of plantar loads during running on different overground surfaces .
	manualset3
248951	2	425483	7	NULL	NULL	0	NULL	plantar loads	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of plantar loads during running on different overground surfaces .
	manualset3
248952	3	425483	7	NULL	NULL	0	NULL	overground surfaces	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of plantar loads during running on different overground surfaces .
	manualset3
248953	4	425483	7	NULL	NULL	0	NULL	running	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of plantar loads during running on different overground surfaces .
	manualset3
248954	1	425484	7	NULL	NULL	0	NULL	Comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of properties of the in vitro and cellular anthramycin-DNA adducts and characterization of the reaction of anthramycin with chromatin .
	manualset3
248955	2	425484	7	NULL	NULL	0	NULL	 properties	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of properties of the in vitro and cellular anthramycin-DNA adducts and characterization of the reaction of anthramycin with chromatin .
	manualset3
248956	3	425484	7	NULL	NULL	0	NULL	cellular anthramycin-DNA adducts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of properties of the in vitro and cellular anthramycin-DNA adducts and characterization of the reaction of anthramycin with chromatin .
	manualset3
248957	4	425484	7	NULL	NULL	0	NULL	characterization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of properties of the in vitro and cellular anthramycin-DNA adducts and characterization of the reaction of anthramycin with chromatin .
	manualset3
248958	5	425484	7	NULL	NULL	0	NULL	reaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of properties of the in vitro and cellular anthramycin-DNA adducts and characterization of the reaction of anthramycin with chromatin .
	manualset3
248959	6	425484	7	NULL	NULL	0	NULL	anthramycin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of properties of the in vitro and cellular anthramycin-DNA adducts and characterization of the reaction of anthramycin with chromatin .
	manualset3
248960	7	425484	7	NULL	NULL	0	NULL	chromatin	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of properties of the in vitro and cellular anthramycin-DNA adducts and characterization of the reaction of anthramycin with chromatin .
	manualset3
248961	1	425485	7	NULL	NULL	0	NULL	Comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of resource utilization and clinical outcomes between teaching and nonteaching medical services .
	manualset3
248962	2	425485	7	NULL	NULL	0	NULL	resource utilization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of resource utilization and clinical outcomes between teaching and nonteaching medical services .
	manualset3
248963	3	425485	7	NULL	NULL	0	NULL	clinical outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of resource utilization and clinical outcomes between teaching and nonteaching medical services .
	manualset3
248964	4	425485	7	NULL	NULL	0	NULL	teaching	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of resource utilization and clinical outcomes between teaching and nonteaching medical services .
	manualset3
248965	5	425485	7	NULL	NULL	0	NULL	nonteaching medical services	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of resource utilization and clinical outcomes between teaching and nonteaching medical services .
	manualset3
248966	1	425486	7	NULL	NULL	0	NULL	Comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the Green scale versus magnitude estimation for taste perception .
	manualset3
248967	2	425486	7	NULL	NULL	0	NULL	Green scale	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the Green scale versus magnitude estimation for taste perception .
	manualset3
248968	3	425486	7	NULL	NULL	0	NULL	magnitude estimation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the Green scale versus magnitude estimation for taste perception .
	manualset3
248969	4	425486	7	NULL	NULL	0	NULL	taste perception	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the Green scale versus magnitude estimation for taste perception .
	manualset3
248970	1	425487	7	NULL	NULL	0	NULL	Comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the Western immunoblot assay and a glycoprotein G enzyme immunoassay for detection of serum antibodies to herpes simplex virus type 2 in patients with AIDS .
	manualset3
248971	2	425487	7	NULL	NULL	0	NULL	Western immunoblot assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the Western immunoblot assay and a glycoprotein G enzyme immunoassay for detection of serum antibodies to herpes simplex virus type 2 in patients with AIDS .
	manualset3
248972	3	425487	7	NULL	NULL	0	NULL	glycoprotein G enzyme immunoassay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the Western immunoblot assay and a glycoprotein G enzyme immunoassay for detection of serum antibodies to herpes simplex virus type 2 in patients with AIDS .
	manualset3
248973	4	425487	7	NULL	NULL	0	NULL	 detection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the Western immunoblot assay and a glycoprotein G enzyme immunoassay for detection of serum antibodies to herpes simplex virus type 2 in patients with AIDS .
	manualset3
248974	5	425487	7	NULL	NULL	0	NULL	serum antibodies	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the Western immunoblot assay and a glycoprotein G enzyme immunoassay for detection of serum antibodies to herpes simplex virus type 2 in patients with AIDS .
	manualset3
248975	6	425487	7	NULL	NULL	0	NULL	herpes simplex virus type 2	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the Western immunoblot assay and a glycoprotein G enzyme immunoassay for detection of serum antibodies to herpes simplex virus type 2 in patients with AIDS .
	manualset3
248976	7	425487	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the Western immunoblot assay and a glycoprotein G enzyme immunoassay for detection of serum antibodies to herpes simplex virus type 2 in patients with AIDS .
	manualset3
248977	8	425487	7	NULL	NULL	0	NULL	AIDS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the Western immunoblot assay and a glycoprotein G enzyme immunoassay for detection of serum antibodies to herpes simplex virus type 2 in patients with AIDS .
	manualset3
248978	1	425488	7	NULL	NULL	0	NULL	Comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the early expression of VGluT genes between the lamprey and some anamniotan gnathostomes ( frog , zebrafish ) reveals a conserved expression pattern , likely to reflect ancestral vertebrate characteristics .
	manualset3
248979	2	425488	7	NULL	NULL	0	NULL	early expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the early expression of VGluT genes between the lamprey and some anamniotan gnathostomes ( frog , zebrafish ) reveals a conserved expression pattern , likely to reflect ancestral vertebrate characteristics .
	manualset3
248980	3	425488	7	NULL	NULL	0	NULL	VGluT genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the early expression of VGluT genes between the lamprey and some anamniotan gnathostomes ( frog , zebrafish ) reveals a conserved expression pattern , likely to reflect ancestral vertebrate characteristics .
	manualset3
248981	4	425488	7	NULL	NULL	0	NULL	lamprey	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the early expression of VGluT genes between the lamprey and some anamniotan gnathostomes ( frog , zebrafish ) reveals a conserved expression pattern , likely to reflect ancestral vertebrate characteristics .
	manualset3
248982	5	425488	7	NULL	NULL	0	NULL	anamniotan gnathostomes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the early expression of VGluT genes between the lamprey and some anamniotan gnathostomes ( frog , zebrafish ) reveals a conserved expression pattern , likely to reflect ancestral vertebrate characteristics .
	manualset3
248983	6	425488	7	NULL	NULL	0	NULL	frog	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the early expression of VGluT genes between the lamprey and some anamniotan gnathostomes ( frog , zebrafish ) reveals a conserved expression pattern , likely to reflect ancestral vertebrate characteristics .
	manualset3
248984	7	425488	7	NULL	NULL	0	NULL	zebrafish	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the early expression of VGluT genes between the lamprey and some anamniotan gnathostomes ( frog , zebrafish ) reveals a conserved expression pattern , likely to reflect ancestral vertebrate characteristics .
	manualset3
248985	8	425488	7	NULL	NULL	0	NULL	conserved expression pattern	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the early expression of VGluT genes between the lamprey and some anamniotan gnathostomes ( frog , zebrafish ) reveals a conserved expression pattern , likely to reflect ancestral vertebrate characteristics .
	manualset3
248986	9	425488	7	NULL	NULL	0	NULL	ancestral vertebrate characteristics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the early expression of VGluT genes between the lamprey and some anamniotan gnathostomes ( frog , zebrafish ) reveals a conserved expression pattern , likely to reflect ancestral vertebrate characteristics .
	manualset3
248987	1	425489	7	NULL	NULL	0	NULL	Comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the transforming gene from 3611-MSV , designated v-raf , with previously isolated retrovirus oncogenes either by direct hybridization or by comparison of restriction fragments of their cellular homologs shows it to be unique .
	manualset3
248988	2	425489	7	NULL	NULL	0	NULL	transforming gene	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the transforming gene from 3611-MSV , designated v-raf , with previously isolated retrovirus oncogenes either by direct hybridization or by comparison of restriction fragments of their cellular homologs shows it to be unique .
	manualset3
248989	3	425489	7	NULL	NULL	0	NULL	3611-MSV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the transforming gene from 3611-MSV , designated v-raf , with previously isolated retrovirus oncogenes either by direct hybridization or by comparison of restriction fragments of their cellular homologs shows it to be unique .
	manualset3
248990	4	425489	7	NULL	NULL	0	NULL	v-raf	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the transforming gene from 3611-MSV , designated v-raf , with previously isolated retrovirus oncogenes either by direct hybridization or by comparison of restriction fragments of their cellular homologs shows it to be unique .
	manualset3
248991	5	425489	7	NULL	NULL	0	NULL	retrovirus oncogenes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the transforming gene from 3611-MSV , designated v-raf , with previously isolated retrovirus oncogenes either by direct hybridization or by comparison of restriction fragments of their cellular homologs shows it to be unique .
	manualset3
248992	6	425489	7	NULL	NULL	0	NULL	direct hybridization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the transforming gene from 3611-MSV , designated v-raf , with previously isolated retrovirus oncogenes either by direct hybridization or by comparison of restriction fragments of their cellular homologs shows it to be unique .
	manualset3
248993	7	425489	7	NULL	NULL	0	NULL	comparison 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the transforming gene from 3611-MSV , designated v-raf , with previously isolated retrovirus oncogenes either by direct hybridization or by comparison of restriction fragments of their cellular homologs shows it to be unique .
	manualset3
248994	8	425489	7	NULL	NULL	0	NULL	restriction fragments 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the transforming gene from 3611-MSV , designated v-raf , with previously isolated retrovirus oncogenes either by direct hybridization or by comparison of restriction fragments of their cellular homologs shows it to be unique .
	manualset3
248995	9	425489	7	NULL	NULL	0	NULL	cellular homologs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of the transforming gene from 3611-MSV , designated v-raf , with previously isolated retrovirus oncogenes either by direct hybridization or by comparison of restriction fragments of their cellular homologs shows it to be unique .
	manualset3
248996	1	425490	7	NULL	NULL	0	NULL	 tricuspid stenosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Isolated tricuspid stenosis ) .
	manualset3
248997	1	425491	7	NULL	NULL	0	NULL	Comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of this technique with HPLC detection of cyclosporin in tears showed a good correlation , with the immunoaffinity CE technique having the advantage of being able to simultaneously detect toxic metabolites of cyclosporin in the same sample .
	manualset3
248998	2	425491	7	NULL	NULL	0	NULL	technique 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of this technique with HPLC detection of cyclosporin in tears showed a good correlation , with the immunoaffinity CE technique having the advantage of being able to simultaneously detect toxic metabolites of cyclosporin in the same sample .
	manualset3
248999	3	425491	7	NULL	NULL	0	NULL	HPLC detection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of this technique with HPLC detection of cyclosporin in tears showed a good correlation , with the immunoaffinity CE technique having the advantage of being able to simultaneously detect toxic metabolites of cyclosporin in the same sample .
	manualset3
249000	4	425491	7	NULL	NULL	0	NULL	 cyclosporin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of this technique with HPLC detection of cyclosporin in tears showed a good correlation , with the immunoaffinity CE technique having the advantage of being able to simultaneously detect toxic metabolites of cyclosporin in the same sample .
	manualset3
249001	5	425491	7	NULL	NULL	0	NULL	 tears	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of this technique with HPLC detection of cyclosporin in tears showed a good correlation , with the immunoaffinity CE technique having the advantage of being able to simultaneously detect toxic metabolites of cyclosporin in the same sample .
	manualset3
249002	6	425491	7	NULL	NULL	0	NULL	good correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of this technique with HPLC detection of cyclosporin in tears showed a good correlation , with the immunoaffinity CE technique having the advantage of being able to simultaneously detect toxic metabolites of cyclosporin in the same sample .
	manualset3
249003	7	425491	7	NULL	NULL	0	NULL	 immunoaffinity CE technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of this technique with HPLC detection of cyclosporin in tears showed a good correlation , with the immunoaffinity CE technique having the advantage of being able to simultaneously detect toxic metabolites of cyclosporin in the same sample .
	manualset3
249004	8	425491	7	NULL	NULL	0	NULL	advantage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of this technique with HPLC detection of cyclosporin in tears showed a good correlation , with the immunoaffinity CE technique having the advantage of being able to simultaneously detect toxic metabolites of cyclosporin in the same sample .
	manualset3
249005	9	425491	7	NULL	NULL	0	NULL	 toxic metabolites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of this technique with HPLC detection of cyclosporin in tears showed a good correlation , with the immunoaffinity CE technique having the advantage of being able to simultaneously detect toxic metabolites of cyclosporin in the same sample .
	manualset3
249006	10	425491	7	NULL	NULL	0	NULL	cyclosporin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of this technique with HPLC detection of cyclosporin in tears showed a good correlation , with the immunoaffinity CE technique having the advantage of being able to simultaneously detect toxic metabolites of cyclosporin in the same sample .
	manualset3
249007	11	425491	7	NULL	NULL	0	NULL	sample	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison of this technique with HPLC detection of cyclosporin in tears showed a good correlation , with the immunoaffinity CE technique having the advantage of being able to simultaneously detect toxic metabolites of cyclosporin in the same sample .
	manualset3
249008	1	425492	7	NULL	NULL	0	NULL	Comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison to control specimens displayed marked restructuralization of the endometrium .
	manualset3
249009	2	425492	7	NULL	NULL	0	NULL	control specimens	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison to control specimens displayed marked restructuralization of the endometrium .
	manualset3
249010	3	425492	7	NULL	NULL	0	NULL	marked restructuralization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison to control specimens displayed marked restructuralization of the endometrium .
	manualset3
249011	4	425492	7	NULL	NULL	0	NULL	endometrium	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison to control specimens displayed marked restructuralization of the endometrium .
	manualset3
249012	1	425493	7	NULL	NULL	0	NULL	Comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with an HPLC method ( x ) showed good agreement : y = 0.98 x + 1.34 , Sy .
	manualset3
249013	2	425493	7	NULL	NULL	0	NULL	HPLC method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with an HPLC method ( x ) showed good agreement : y = 0.98 x + 1.34 , Sy .
	manualset3
249014	3	425493	7	NULL	NULL	0	NULL	good agreement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with an HPLC method ( x ) showed good agreement : y = 0.98 x + 1.34 , Sy .
	manualset3
249015	4	425493	7	NULL	NULL	0	NULL	y = 0.98 x + 1.34 , Sy	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with an HPLC method ( x ) showed good agreement : y = 0.98 x + 1.34 , Sy .
	manualset3
249016	1	425494	7	NULL	NULL	0	NULL	Comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with cefazolin , cefoxitin and cefamandole ( author 's transl ) ) .
	manualset3
249017	2	425494	7	NULL	NULL	0	NULL	cefazolin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with cefazolin , cefoxitin and cefamandole ( author 's transl ) ) .
	manualset3
249018	3	425494	7	NULL	NULL	0	NULL	cefoxitin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with cefazolin , cefoxitin and cefamandole ( author 's transl ) ) .
	manualset3
249019	4	425494	7	NULL	NULL	0	NULL	cefamandole 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with cefazolin , cefoxitin and cefamandole ( author 's transl ) ) .
	manualset3
249020	5	425494	7	NULL	NULL	0	NULL	 author 's transl 	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with cefazolin , cefoxitin and cefamandole ( author 's transl ) ) .
	manualset3
249021	1	425495	7	NULL	NULL	0	NULL	Comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with five published global studies reveals that these Australians demonstrate greatest divergence from some Africans , least from Papua New Guinea ( PNG ) highlanders , and only slightly more divergence from some Pacific groups ( Indonesian , Asian , Samoan , and coastal PNG ) .
	manualset3
249022	2	425495	7	NULL	NULL	0	NULL	five published global studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with five published global studies reveals that these Australians demonstrate greatest divergence from some Africans , least from Papua New Guinea ( PNG ) highlanders , and only slightly more divergence from some Pacific groups ( Indonesian , Asian , Samoan , and coastal PNG ) .
	manualset3
249023	3	425495	7	NULL	NULL	0	NULL	Australians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with five published global studies reveals that these Australians demonstrate greatest divergence from some Africans , least from Papua New Guinea ( PNG ) highlanders , and only slightly more divergence from some Pacific groups ( Indonesian , Asian , Samoan , and coastal PNG ) .
	manualset3
249024	4	425495	7	NULL	NULL	0	NULL	greatest divergence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with five published global studies reveals that these Australians demonstrate greatest divergence from some Africans , least from Papua New Guinea ( PNG ) highlanders , and only slightly more divergence from some Pacific groups ( Indonesian , Asian , Samoan , and coastal PNG ) .
	manualset3
249025	5	425495	7	NULL	NULL	0	NULL	Africans	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with five published global studies reveals that these Australians demonstrate greatest divergence from some Africans , least from Papua New Guinea ( PNG ) highlanders , and only slightly more divergence from some Pacific groups ( Indonesian , Asian , Samoan , and coastal PNG ) .
	manualset3
249026	6	425495	7	NULL	NULL	0	NULL	Papua New Guinea ( PNG ) highlanders	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with five published global studies reveals that these Australians demonstrate greatest divergence from some Africans , least from Papua New Guinea ( PNG ) highlanders , and only slightly more divergence from some Pacific groups ( Indonesian , Asian , Samoan , and coastal PNG ) .
	manualset3
249027	7	425495	7	NULL	NULL	0	NULL	divergence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with five published global studies reveals that these Australians demonstrate greatest divergence from some Africans , least from Papua New Guinea ( PNG ) highlanders , and only slightly more divergence from some Pacific groups ( Indonesian , Asian , Samoan , and coastal PNG ) .
	manualset3
249028	8	425495	7	NULL	NULL	0	NULL	Pacific groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with five published global studies reveals that these Australians demonstrate greatest divergence from some Africans , least from Papua New Guinea ( PNG ) highlanders , and only slightly more divergence from some Pacific groups ( Indonesian , Asian , Samoan , and coastal PNG ) .
	manualset3
249029	9	425495	7	NULL	NULL	0	NULL	Indonesian	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with five published global studies reveals that these Australians demonstrate greatest divergence from some Africans , least from Papua New Guinea ( PNG ) highlanders , and only slightly more divergence from some Pacific groups ( Indonesian , Asian , Samoan , and coastal PNG ) .
	manualset3
249030	10	425495	7	NULL	NULL	0	NULL	Asian	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with five published global studies reveals that these Australians demonstrate greatest divergence from some Africans , least from Papua New Guinea ( PNG ) highlanders , and only slightly more divergence from some Pacific groups ( Indonesian , Asian , Samoan , and coastal PNG ) .
	manualset3
249031	11	425495	7	NULL	NULL	0	NULL	 Samoan	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with five published global studies reveals that these Australians demonstrate greatest divergence from some Africans , least from Papua New Guinea ( PNG ) highlanders , and only slightly more divergence from some Pacific groups ( Indonesian , Asian , Samoan , and coastal PNG ) .
	manualset3
249032	12	425495	7	NULL	NULL	0	NULL	coastal PNG	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with five published global studies reveals that these Australians demonstrate greatest divergence from some Africans , least from Papua New Guinea ( PNG ) highlanders , and only slightly more divergence from some Pacific groups ( Indonesian , Asian , Samoan , and coastal PNG ) .
	manualset3
249033	1	425496	7	NULL	NULL	0	NULL	Comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with potentiations evoked at different strengths in control solution suggested that much , but not all , of the increased decay rate observed in the presence of staurosporine could be explained by an impared induction .
	manualset3
249034	2	425496	7	NULL	NULL	0	NULL	potentiations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with potentiations evoked at different strengths in control solution suggested that much , but not all , of the increased decay rate observed in the presence of staurosporine could be explained by an impared induction .
	manualset3
249035	3	425496	7	NULL	NULL	0	NULL	different strengths	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with potentiations evoked at different strengths in control solution suggested that much , but not all , of the increased decay rate observed in the presence of staurosporine could be explained by an impared induction .
	manualset3
249036	4	425496	7	NULL	NULL	0	NULL	control solution 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with potentiations evoked at different strengths in control solution suggested that much , but not all , of the increased decay rate observed in the presence of staurosporine could be explained by an impared induction .
	manualset3
249037	5	425496	7	NULL	NULL	0	NULL	increased decay rate	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with potentiations evoked at different strengths in control solution suggested that much , but not all , of the increased decay rate observed in the presence of staurosporine could be explained by an impared induction .
	manualset3
249038	6	425496	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with potentiations evoked at different strengths in control solution suggested that much , but not all , of the increased decay rate observed in the presence of staurosporine could be explained by an impared induction .
	manualset3
249039	7	425496	7	NULL	NULL	0	NULL	staurosporine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with potentiations evoked at different strengths in control solution suggested that much , but not all , of the increased decay rate observed in the presence of staurosporine could be explained by an impared induction .
	manualset3
249040	8	425496	7	NULL	NULL	0	NULL	impared induction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with potentiations evoked at different strengths in control solution suggested that much , but not all , of the increased decay rate observed in the presence of staurosporine could be explained by an impared induction .
	manualset3
249041	1	425497	7	NULL	NULL	0	NULL	Comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with results from classical trajectory calculations highlights the need of a quantum description of the dynamics in the astrophysically relevant energy range , whereas preliminary results of an extensive first-principles investigation of the reaction energetics reveal the importance of the adopted substrate model .
	manualset3
249042	2	425497	7	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with results from classical trajectory calculations highlights the need of a quantum description of the dynamics in the astrophysically relevant energy range , whereas preliminary results of an extensive first-principles investigation of the reaction energetics reveal the importance of the adopted substrate model .
	manualset3
249043	3	425497	7	NULL	NULL	0	NULL	classical trajectory calculations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with results from classical trajectory calculations highlights the need of a quantum description of the dynamics in the astrophysically relevant energy range , whereas preliminary results of an extensive first-principles investigation of the reaction energetics reveal the importance of the adopted substrate model .
	manualset3
249044	4	425497	7	NULL	NULL	0	NULL	 quantum description	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with results from classical trajectory calculations highlights the need of a quantum description of the dynamics in the astrophysically relevant energy range , whereas preliminary results of an extensive first-principles investigation of the reaction energetics reveal the importance of the adopted substrate model .
	manualset3
249045	5	425497	7	NULL	NULL	0	NULL	dynamics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with results from classical trajectory calculations highlights the need of a quantum description of the dynamics in the astrophysically relevant energy range , whereas preliminary results of an extensive first-principles investigation of the reaction energetics reveal the importance of the adopted substrate model .
	manualset3
249046	6	425497	7	NULL	NULL	0	NULL	energy range	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with results from classical trajectory calculations highlights the need of a quantum description of the dynamics in the astrophysically relevant energy range , whereas preliminary results of an extensive first-principles investigation of the reaction energetics reveal the importance of the adopted substrate model .
	manualset3
249047	7	425497	7	NULL	NULL	0	NULL	preliminary results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with results from classical trajectory calculations highlights the need of a quantum description of the dynamics in the astrophysically relevant energy range , whereas preliminary results of an extensive first-principles investigation of the reaction energetics reveal the importance of the adopted substrate model .
	manualset3
249048	8	425497	7	NULL	NULL	0	NULL	 first-principles investigation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with results from classical trajectory calculations highlights the need of a quantum description of the dynamics in the astrophysically relevant energy range , whereas preliminary results of an extensive first-principles investigation of the reaction energetics reveal the importance of the adopted substrate model .
	manualset3
249049	9	425497	7	NULL	NULL	0	NULL	reaction energetics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with results from classical trajectory calculations highlights the need of a quantum description of the dynamics in the astrophysically relevant energy range , whereas preliminary results of an extensive first-principles investigation of the reaction energetics reveal the importance of the adopted substrate model .
	manualset3
249050	10	425497	7	NULL	NULL	0	NULL	adopted substrate model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparison with results from classical trajectory calculations highlights the need of a quantum description of the dynamics in the astrophysically relevant energy range , whereas preliminary results of an extensive first-principles investigation of the reaction energetics reveal the importance of the adopted substrate model .
	manualset3
249051	1	425498	7	NULL	NULL	0	NULL	Comparisons	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparisons between patients and control values showed a significant decrease in total plasma tryptophan and platelet 5-HT in unmedicated patients .
	manualset3
249052	2	425498	7	NULL	NULL	0	NULL	patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparisons between patients and control values showed a significant decrease in total plasma tryptophan and platelet 5-HT in unmedicated patients .
	manualset3
249053	3	425498	7	NULL	NULL	0	NULL	control values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparisons between patients and control values showed a significant decrease in total plasma tryptophan and platelet 5-HT in unmedicated patients .
	manualset3
249054	4	425498	7	NULL	NULL	0	NULL	total plasma tryptophan	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparisons between patients and control values showed a significant decrease in total plasma tryptophan and platelet 5-HT in unmedicated patients .
	manualset3
249055	5	425498	7	NULL	NULL	0	NULL	platelet 5-HT	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparisons between patients and control values showed a significant decrease in total plasma tryptophan and platelet 5-HT in unmedicated patients .
	manualset3
249056	6	425498	7	NULL	NULL	0	NULL	unmedicated patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparisons between patients and control values showed a significant decrease in total plasma tryptophan and platelet 5-HT in unmedicated patients .
	manualset3
249057	1	425499	7	NULL	NULL	0	NULL	Isolation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Isolation of mesenchymal stem cells from human umbilical cord blood and its bone inducing activity in vitro ) .
	manualset3
249058	2	425499	7	NULL	NULL	0	NULL	mesenchymal stem cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	( Isolation of mesenchymal stem cells from human umbilical cord blood and its bone inducing activity in vitro ) .
	manualset3
249059	3	425499	7	NULL	NULL	0	NULL	human umbilical cord blood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Isolation of mesenchymal stem cells from human umbilical cord blood and its bone inducing activity in vitro ) .
	manualset3
249060	4	425499	7	NULL	NULL	NULL	NULL	bone inducing activity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Isolation of mesenchymal stem cells from human umbilical cord blood and its bone inducing activity in vitro ) .
	manualset3
249061	1	425500	7	NULL	NULL	0	NULL	Comparisons 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparisons of L-type current activity were made using dialyzed , whole-cell voltage-clamp techniques and Ba2 + as charge carrier .
	manualset3
249062	2	425500	7	NULL	NULL	0	NULL	L-type current activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparisons of L-type current activity were made using dialyzed , whole-cell voltage-clamp techniques and Ba2 + as charge carrier .
	manualset3
249063	3	425500	7	NULL	NULL	0	NULL	whole-cell voltage-clamp techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparisons of L-type current activity were made using dialyzed , whole-cell voltage-clamp techniques and Ba2 + as charge carrier .
	manualset3
249064	4	425500	7	NULL	NULL	0	NULL	Ba2 +	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparisons of L-type current activity were made using dialyzed , whole-cell voltage-clamp techniques and Ba2 + as charge carrier .
	manualset3
249065	5	425500	7	NULL	NULL	0	NULL	charge carrier	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparisons of L-type current activity were made using dialyzed , whole-cell voltage-clamp techniques and Ba2 + as charge carrier .
	manualset3
249066	1	425501	7	NULL	NULL	0	NULL	Comparisons 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparisons with films of pure hexanol and pentanoic acid/hexanol mixtures indicate that surface OH groups are more effective than COOH groups in catalyzing HCl entry .
	manualset3
249067	2	425501	7	NULL	NULL	0	NULL	films	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparisons with films of pure hexanol and pentanoic acid/hexanol mixtures indicate that surface OH groups are more effective than COOH groups in catalyzing HCl entry .
	manualset3
249068	3	425501	7	NULL	NULL	0	NULL	pure hexanol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparisons with films of pure hexanol and pentanoic acid/hexanol mixtures indicate that surface OH groups are more effective than COOH groups in catalyzing HCl entry .
	manualset3
249069	4	425501	7	NULL	NULL	0	NULL	pentanoic acid/hexanol mixtures 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparisons with films of pure hexanol and pentanoic acid/hexanol mixtures indicate that surface OH groups are more effective than COOH groups in catalyzing HCl entry .
	manualset3
249070	5	425501	7	NULL	NULL	0	NULL	surface OH groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparisons with films of pure hexanol and pentanoic acid/hexanol mixtures indicate that surface OH groups are more effective than COOH groups in catalyzing HCl entry .
	manualset3
249071	6	425501	7	NULL	NULL	0	NULL	COOH groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparisons with films of pure hexanol and pentanoic acid/hexanol mixtures indicate that surface OH groups are more effective than COOH groups in catalyzing HCl entry .
	manualset3
249072	7	425501	7	NULL	NULL	0	NULL	HCl entry	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Comparisons with films of pure hexanol and pentanoic acid/hexanol mixtures indicate that surface OH groups are more effective than COOH groups in catalyzing HCl entry .
	manualset3
249073	1	425502	7	NULL	NULL	0	NULL	Compartment pressures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compartment pressures after submuscular fixation of proximal tibia fractures .
	manualset3
249074	2	425502	7	NULL	NULL	0	NULL	submuscular fixation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compartment pressures after submuscular fixation of proximal tibia fractures .
	manualset3
249075	3	425502	7	NULL	NULL	0	NULL	proximal tibia fractures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Compartment pressures after submuscular fixation of proximal tibia fractures .
	manualset3
249076	1	425503	7	NULL	NULL	0	NULL	Compartment syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Compartment syndrome from balloon pump .
	manualset3
249077	2	425503	7	NULL	NULL	0	NULL	balloon pump	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Compartment syndrome from balloon pump .
	manualset3
249078	1	425504	7	NULL	NULL	0	NULL	Compensation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compensation of pulse-distortion in saturated laser amplifiers .
	manualset3
249079	2	425504	7	NULL	NULL	0	NULL	pulse-distortion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compensation of pulse-distortion in saturated laser amplifiers .
	manualset3
249080	3	425504	7	NULL	NULL	0	NULL	saturated laser amplifiers	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Compensation of pulse-distortion in saturated laser amplifiers .
	manualset3
249081	1	425505	7	NULL	NULL	0	NULL	Compensatory adrenal growth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Compensatory adrenal growth in relation to stress of surgery and estradiol in adult male rats .
	manualset3
249082	2	425505	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Compensatory adrenal growth in relation to stress of surgery and estradiol in adult male rats .
	manualset3
249083	3	425505	7	NULL	NULL	0	NULL	 stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Compensatory adrenal growth in relation to stress of surgery and estradiol in adult male rats .
	manualset3
249084	4	425505	7	NULL	NULL	0	NULL	surgery 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Compensatory adrenal growth in relation to stress of surgery and estradiol in adult male rats .
	manualset3
249085	5	425505	7	NULL	NULL	0	NULL	estradiol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compensatory adrenal growth in relation to stress of surgery and estradiol in adult male rats .
	manualset3
249086	6	425505	7	NULL	NULL	0	NULL	adult male rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Compensatory adrenal growth in relation to stress of surgery and estradiol in adult male rats .
	manualset3
249087	1	425506	7	NULL	NULL	0	NULL	Competition assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Competition assays with peptide-epoxide scanning libraries revealed common and unique inhibitory fingerprints .
	manualset3
249088	2	425506	7	NULL	NULL	0	NULL	peptide-epoxide scanning libraries	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Competition assays with peptide-epoxide scanning libraries revealed common and unique inhibitory fingerprints .
	manualset3
249089	3	425506	7	NULL	NULL	0	NULL	unique inhibitory fingerprints	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Competition assays with peptide-epoxide scanning libraries revealed common and unique inhibitory fingerprints .
	manualset3
249090	1	425507	7	NULL	NULL	0	NULL	Isomeric derivatives	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Isomeric derivatives of lupinine and epilupinine -- organophosphorus inhibitors of cholinesterases ) .
	manualset3
249091	2	425507	7	NULL	NULL	0	NULL	lupinine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Isomeric derivatives of lupinine and epilupinine -- organophosphorus inhibitors of cholinesterases ) .
	manualset3
249092	3	425507	7	NULL	NULL	0	NULL	epilupinine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Isomeric derivatives of lupinine and epilupinine -- organophosphorus inhibitors of cholinesterases ) .
	manualset3
249093	4	425507	7	NULL	NULL	0	NULL	 organophosphorus inhibitors 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Isomeric derivatives of lupinine and epilupinine -- organophosphorus inhibitors of cholinesterases ) .
	manualset3
249094	5	425507	7	NULL	NULL	0	NULL	cholinesterases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Isomeric derivatives of lupinine and epilupinine -- organophosphorus inhibitors of cholinesterases ) .
	manualset3
249292	1	425508	7	NULL	NULL	0	NULL	Competitive binding studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive binding studies with excess unlabelled Ft significantly reduced binding , and uptake studies at 37 degrees C showed saturation after 4 h. Enhancing and blocking endocytosis using Mas-7 ( a G-protein activator ) and hypertonic medium ( 0.5 M sucrose ) , respectively , demonstrated that Ft-Fe uptake by Mas-7-treated cells was 140 % of control cells , whereas sucrose treatment resulted in a statistically significant reduction in Ft-Fe uptake by 70 % as compared to controls .
	manualset3
249293	2	425508	7	NULL	NULL	0	NULL	excess unlabelled Ft 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive binding studies with excess unlabelled Ft significantly reduced binding , and uptake studies at 37 degrees C showed saturation after 4 h. Enhancing and blocking endocytosis using Mas-7 ( a G-protein activator ) and hypertonic medium ( 0.5 M sucrose ) , respectively , demonstrated that Ft-Fe uptake by Mas-7-treated cells was 140 % of control cells , whereas sucrose treatment resulted in a statistically significant reduction in Ft-Fe uptake by 70 % as compared to controls .
	manualset3
249294	3	425508	7	NULL	NULL	0	NULL	binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive binding studies with excess unlabelled Ft significantly reduced binding , and uptake studies at 37 degrees C showed saturation after 4 h. Enhancing and blocking endocytosis using Mas-7 ( a G-protein activator ) and hypertonic medium ( 0.5 M sucrose ) , respectively , demonstrated that Ft-Fe uptake by Mas-7-treated cells was 140 % of control cells , whereas sucrose treatment resulted in a statistically significant reduction in Ft-Fe uptake by 70 % as compared to controls .
	manualset3
249295	4	425508	7	NULL	NULL	0	NULL	uptake studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive binding studies with excess unlabelled Ft significantly reduced binding , and uptake studies at 37 degrees C showed saturation after 4 h. Enhancing and blocking endocytosis using Mas-7 ( a G-protein activator ) and hypertonic medium ( 0.5 M sucrose ) , respectively , demonstrated that Ft-Fe uptake by Mas-7-treated cells was 140 % of control cells , whereas sucrose treatment resulted in a statistically significant reduction in Ft-Fe uptake by 70 % as compared to controls .
	manualset3
249296	5	425508	7	NULL	NULL	0	NULL	37 degrees C	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive binding studies with excess unlabelled Ft significantly reduced binding , and uptake studies at 37 degrees C showed saturation after 4 h. Enhancing and blocking endocytosis using Mas-7 ( a G-protein activator ) and hypertonic medium ( 0.5 M sucrose ) , respectively , demonstrated that Ft-Fe uptake by Mas-7-treated cells was 140 % of control cells , whereas sucrose treatment resulted in a statistically significant reduction in Ft-Fe uptake by 70 % as compared to controls .
	manualset3
249297	6	425508	7	NULL	NULL	0	NULL	saturation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive binding studies with excess unlabelled Ft significantly reduced binding , and uptake studies at 37 degrees C showed saturation after 4 h. Enhancing and blocking endocytosis using Mas-7 ( a G-protein activator ) and hypertonic medium ( 0.5 M sucrose ) , respectively , demonstrated that Ft-Fe uptake by Mas-7-treated cells was 140 % of control cells , whereas sucrose treatment resulted in a statistically significant reduction in Ft-Fe uptake by 70 % as compared to controls .
	manualset3
249298	7	425508	7	NULL	NULL	0	NULL	4 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive binding studies with excess unlabelled Ft significantly reduced binding , and uptake studies at 37 degrees C showed saturation after 4 h. Enhancing and blocking endocytosis using Mas-7 ( a G-protein activator ) and hypertonic medium ( 0.5 M sucrose ) , respectively , demonstrated that Ft-Fe uptake by Mas-7-treated cells was 140 % of control cells , whereas sucrose treatment resulted in a statistically significant reduction in Ft-Fe uptake by 70 % as compared to controls .
	manualset3
249299	8	425508	7	NULL	NULL	0	NULL	endocytosis 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive binding studies with excess unlabelled Ft significantly reduced binding , and uptake studies at 37 degrees C showed saturation after 4 h. Enhancing and blocking endocytosis using Mas-7 ( a G-protein activator ) and hypertonic medium ( 0.5 M sucrose ) , respectively , demonstrated that Ft-Fe uptake by Mas-7-treated cells was 140 % of control cells , whereas sucrose treatment resulted in a statistically significant reduction in Ft-Fe uptake by 70 % as compared to controls .
	manualset3
249300	9	425508	7	NULL	NULL	0	NULL	Mas-7	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive binding studies with excess unlabelled Ft significantly reduced binding , and uptake studies at 37 degrees C showed saturation after 4 h. Enhancing and blocking endocytosis using Mas-7 ( a G-protein activator ) and hypertonic medium ( 0.5 M sucrose ) , respectively , demonstrated that Ft-Fe uptake by Mas-7-treated cells was 140 % of control cells , whereas sucrose treatment resulted in a statistically significant reduction in Ft-Fe uptake by 70 % as compared to controls .
	manualset3
249301	10	425508	7	NULL	NULL	0	NULL	G-protein activator	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive binding studies with excess unlabelled Ft significantly reduced binding , and uptake studies at 37 degrees C showed saturation after 4 h. Enhancing and blocking endocytosis using Mas-7 ( a G-protein activator ) and hypertonic medium ( 0.5 M sucrose ) , respectively , demonstrated that Ft-Fe uptake by Mas-7-treated cells was 140 % of control cells , whereas sucrose treatment resulted in a statistically significant reduction in Ft-Fe uptake by 70 % as compared to controls .
	manualset3
249302	11	425508	7	NULL	NULL	0	NULL	hypertonic medium	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive binding studies with excess unlabelled Ft significantly reduced binding , and uptake studies at 37 degrees C showed saturation after 4 h. Enhancing and blocking endocytosis using Mas-7 ( a G-protein activator ) and hypertonic medium ( 0.5 M sucrose ) , respectively , demonstrated that Ft-Fe uptake by Mas-7-treated cells was 140 % of control cells , whereas sucrose treatment resulted in a statistically significant reduction in Ft-Fe uptake by 70 % as compared to controls .
	manualset3
249303	12	425508	7	NULL	NULL	0	NULL	 0.5 M sucrose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive binding studies with excess unlabelled Ft significantly reduced binding , and uptake studies at 37 degrees C showed saturation after 4 h. Enhancing and blocking endocytosis using Mas-7 ( a G-protein activator ) and hypertonic medium ( 0.5 M sucrose ) , respectively , demonstrated that Ft-Fe uptake by Mas-7-treated cells was 140 % of control cells , whereas sucrose treatment resulted in a statistically significant reduction in Ft-Fe uptake by 70 % as compared to controls .
	manualset3
249304	13	425508	7	NULL	NULL	0	NULL	Ft-Fe uptake	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive binding studies with excess unlabelled Ft significantly reduced binding , and uptake studies at 37 degrees C showed saturation after 4 h. Enhancing and blocking endocytosis using Mas-7 ( a G-protein activator ) and hypertonic medium ( 0.5 M sucrose ) , respectively , demonstrated that Ft-Fe uptake by Mas-7-treated cells was 140 % of control cells , whereas sucrose treatment resulted in a statistically significant reduction in Ft-Fe uptake by 70 % as compared to controls .
	manualset3
249305	14	425508	7	NULL	NULL	0	NULL	Mas-7-treated cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive binding studies with excess unlabelled Ft significantly reduced binding , and uptake studies at 37 degrees C showed saturation after 4 h. Enhancing and blocking endocytosis using Mas-7 ( a G-protein activator ) and hypertonic medium ( 0.5 M sucrose ) , respectively , demonstrated that Ft-Fe uptake by Mas-7-treated cells was 140 % of control cells , whereas sucrose treatment resulted in a statistically significant reduction in Ft-Fe uptake by 70 % as compared to controls .
	manualset3
249306	15	425508	7	NULL	NULL	0	NULL	140 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive binding studies with excess unlabelled Ft significantly reduced binding , and uptake studies at 37 degrees C showed saturation after 4 h. Enhancing and blocking endocytosis using Mas-7 ( a G-protein activator ) and hypertonic medium ( 0.5 M sucrose ) , respectively , demonstrated that Ft-Fe uptake by Mas-7-treated cells was 140 % of control cells , whereas sucrose treatment resulted in a statistically significant reduction in Ft-Fe uptake by 70 % as compared to controls .
	manualset3
249307	16	425508	7	NULL	NULL	0	NULL	control cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive binding studies with excess unlabelled Ft significantly reduced binding , and uptake studies at 37 degrees C showed saturation after 4 h. Enhancing and blocking endocytosis using Mas-7 ( a G-protein activator ) and hypertonic medium ( 0.5 M sucrose ) , respectively , demonstrated that Ft-Fe uptake by Mas-7-treated cells was 140 % of control cells , whereas sucrose treatment resulted in a statistically significant reduction in Ft-Fe uptake by 70 % as compared to controls .
	manualset3
249308	17	425508	7	NULL	NULL	0	NULL	sucrose treatment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive binding studies with excess unlabelled Ft significantly reduced binding , and uptake studies at 37 degrees C showed saturation after 4 h. Enhancing and blocking endocytosis using Mas-7 ( a G-protein activator ) and hypertonic medium ( 0.5 M sucrose ) , respectively , demonstrated that Ft-Fe uptake by Mas-7-treated cells was 140 % of control cells , whereas sucrose treatment resulted in a statistically significant reduction in Ft-Fe uptake by 70 % as compared to controls .
	manualset3
249309	18	425508	7	NULL	NULL	0	NULL	reduction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive binding studies with excess unlabelled Ft significantly reduced binding , and uptake studies at 37 degrees C showed saturation after 4 h. Enhancing and blocking endocytosis using Mas-7 ( a G-protein activator ) and hypertonic medium ( 0.5 M sucrose ) , respectively , demonstrated that Ft-Fe uptake by Mas-7-treated cells was 140 % of control cells , whereas sucrose treatment resulted in a statistically significant reduction in Ft-Fe uptake by 70 % as compared to controls .
	manualset3
249310	19	425508	7	NULL	NULL	0	NULL	Ft-Fe uptake	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive binding studies with excess unlabelled Ft significantly reduced binding , and uptake studies at 37 degrees C showed saturation after 4 h. Enhancing and blocking endocytosis using Mas-7 ( a G-protein activator ) and hypertonic medium ( 0.5 M sucrose ) , respectively , demonstrated that Ft-Fe uptake by Mas-7-treated cells was 140 % of control cells , whereas sucrose treatment resulted in a statistically significant reduction in Ft-Fe uptake by 70 % as compared to controls .
	manualset3
249311	20	425508	7	NULL	NULL	0	NULL	70 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive binding studies with excess unlabelled Ft significantly reduced binding , and uptake studies at 37 degrees C showed saturation after 4 h. Enhancing and blocking endocytosis using Mas-7 ( a G-protein activator ) and hypertonic medium ( 0.5 M sucrose ) , respectively , demonstrated that Ft-Fe uptake by Mas-7-treated cells was 140 % of control cells , whereas sucrose treatment resulted in a statistically significant reduction in Ft-Fe uptake by 70 % as compared to controls .
	manualset3
249312	21	425508	7	NULL	NULL	0	NULL	controls	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive binding studies with excess unlabelled Ft significantly reduced binding , and uptake studies at 37 degrees C showed saturation after 4 h. Enhancing and blocking endocytosis using Mas-7 ( a G-protein activator ) and hypertonic medium ( 0.5 M sucrose ) , respectively , demonstrated that Ft-Fe uptake by Mas-7-treated cells was 140 % of control cells , whereas sucrose treatment resulted in a statistically significant reduction in Ft-Fe uptake by 70 % as compared to controls .
	manualset3
249313	1	425509	7	NULL	NULL	0	NULL	Competitive inhibition experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive inhibition experiments suggest the presence of at least two transport systems : a Na + - independent , pH-insensitive system inhibitable by cationic amino acids , similar to system y + , and a Na + - dependent system which recognizes both cationic and neutral amino acids only in the presence of Na + , i.e. a Bo , + - like system .
	manualset3
249314	2	425509	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive inhibition experiments suggest the presence of at least two transport systems : a Na + - independent , pH-insensitive system inhibitable by cationic amino acids , similar to system y + , and a Na + - dependent system which recognizes both cationic and neutral amino acids only in the presence of Na + , i.e. a Bo , + - like system .
	manualset3
249315	3	425509	7	NULL	NULL	0	NULL	two transport systems	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive inhibition experiments suggest the presence of at least two transport systems : a Na + - independent , pH-insensitive system inhibitable by cationic amino acids , similar to system y + , and a Na + - dependent system which recognizes both cationic and neutral amino acids only in the presence of Na + , i.e. a Bo , + - like system .
	manualset3
249316	4	425509	7	NULL	NULL	0	NULL	Na + - independent system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive inhibition experiments suggest the presence of at least two transport systems : a Na + - independent , pH-insensitive system inhibitable by cationic amino acids , similar to system y + , and a Na + - dependent system which recognizes both cationic and neutral amino acids only in the presence of Na + , i.e. a Bo , + - like system .
	manualset3
249317	5	425509	7	NULL	NULL	0	NULL	 pH-insensitive system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive inhibition experiments suggest the presence of at least two transport systems : a Na + - independent , pH-insensitive system inhibitable by cationic amino acids , similar to system y + , and a Na + - dependent system which recognizes both cationic and neutral amino acids only in the presence of Na + , i.e. a Bo , + - like system .
	manualset3
249318	6	425509	7	NULL	NULL	0	NULL	cationic amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive inhibition experiments suggest the presence of at least two transport systems : a Na + - independent , pH-insensitive system inhibitable by cationic amino acids , similar to system y + , and a Na + - dependent system which recognizes both cationic and neutral amino acids only in the presence of Na + , i.e. a Bo , + - like system .
	manualset3
249319	7	425509	7	NULL	NULL	0	NULL	y +	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive inhibition experiments suggest the presence of at least two transport systems : a Na + - independent , pH-insensitive system inhibitable by cationic amino acids , similar to system y + , and a Na + - dependent system which recognizes both cationic and neutral amino acids only in the presence of Na + , i.e. a Bo , + - like system .
	manualset3
249320	8	425509	7	NULL	NULL	0	NULL	Na + - dependent system 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive inhibition experiments suggest the presence of at least two transport systems : a Na + - independent , pH-insensitive system inhibitable by cationic amino acids , similar to system y + , and a Na + - dependent system which recognizes both cationic and neutral amino acids only in the presence of Na + , i.e. a Bo , + - like system .
	manualset3
249321	9	425509	7	NULL	NULL	0	NULL	cationic amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive inhibition experiments suggest the presence of at least two transport systems : a Na + - independent , pH-insensitive system inhibitable by cationic amino acids , similar to system y + , and a Na + - dependent system which recognizes both cationic and neutral amino acids only in the presence of Na + , i.e. a Bo , + - like system .
	manualset3
249322	10	425509	7	NULL	NULL	0	NULL	neutral amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive inhibition experiments suggest the presence of at least two transport systems : a Na + - independent , pH-insensitive system inhibitable by cationic amino acids , similar to system y + , and a Na + - dependent system which recognizes both cationic and neutral amino acids only in the presence of Na + , i.e. a Bo , + - like system .
	manualset3
249323	11	425509	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive inhibition experiments suggest the presence of at least two transport systems : a Na + - independent , pH-insensitive system inhibitable by cationic amino acids , similar to system y + , and a Na + - dependent system which recognizes both cationic and neutral amino acids only in the presence of Na + , i.e. a Bo , + - like system .
	manualset3
249324	12	425509	7	NULL	NULL	0	NULL	Na +	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive inhibition experiments suggest the presence of at least two transport systems : a Na + - independent , pH-insensitive system inhibitable by cationic amino acids , similar to system y + , and a Na + - dependent system which recognizes both cationic and neutral amino acids only in the presence of Na + , i.e. a Bo , + - like system .
	manualset3
249325	13	425509	7	NULL	NULL	0	NULL	Bo , + - like system	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive inhibition experiments suggest the presence of at least two transport systems : a Na + - independent , pH-insensitive system inhibitable by cationic amino acids , similar to system y + , and a Na + - dependent system which recognizes both cationic and neutral amino acids only in the presence of Na + , i.e. a Bo , + - like system .
	manualset3
249326	1	425510	7	NULL	NULL	0	NULL	Competitive inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive inhibition was found for the MSE-treated CYP2D6 inhibition assay , whereas non-competitive inhibition was shown in inhibition assays using CYP3A4 , CYP1A2 and CYP2C19 .
	manualset3
249327	2	425510	7	NULL	NULL	0	NULL	MSE-treated CYP2D6 inhibition assay 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive inhibition was found for the MSE-treated CYP2D6 inhibition assay , whereas non-competitive inhibition was shown in inhibition assays using CYP3A4 , CYP1A2 and CYP2C19 .
	manualset3
249328	3	425510	7	NULL	NULL	0	NULL	non-competitive inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive inhibition was found for the MSE-treated CYP2D6 inhibition assay , whereas non-competitive inhibition was shown in inhibition assays using CYP3A4 , CYP1A2 and CYP2C19 .
	manualset3
249329	4	425510	7	NULL	NULL	0	NULL	 inhibition assays 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive inhibition was found for the MSE-treated CYP2D6 inhibition assay , whereas non-competitive inhibition was shown in inhibition assays using CYP3A4 , CYP1A2 and CYP2C19 .
	manualset3
249330	5	425510	7	NULL	NULL	0	NULL	CYP3A4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive inhibition was found for the MSE-treated CYP2D6 inhibition assay , whereas non-competitive inhibition was shown in inhibition assays using CYP3A4 , CYP1A2 and CYP2C19 .
	manualset3
249331	6	425510	7	NULL	NULL	0	NULL	CYP1A2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive inhibition was found for the MSE-treated CYP2D6 inhibition assay , whereas non-competitive inhibition was shown in inhibition assays using CYP3A4 , CYP1A2 and CYP2C19 .
	manualset3
249332	7	425510	7	NULL	NULL	0	NULL	CYP2C19 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Competitive inhibition was found for the MSE-treated CYP2D6 inhibition assay , whereas non-competitive inhibition was shown in inhibition assays using CYP3A4 , CYP1A2 and CYP2C19 .
	manualset3
249333	1	425511	7	NULL	NULL	0	NULL	Complement-fixation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Complement-fixation in experimental and human poliomyelitis .
	manualset3
249334	2	425511	7	NULL	NULL	0	NULL	human poliomyelitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Complement-fixation in experimental and human poliomyelitis .
	manualset3
249335	1	425512	7	NULL	NULL	0	NULL	Complement activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Complement activity and C3 levels in Crry ( - / - ) mice were markedly reduced .
	manualset3
249336	2	425512	7	NULL	NULL	0	NULL	C3 levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Complement activity and C3 levels in Crry ( - / - ) mice were markedly reduced .
	manualset3
249337	3	425512	7	NULL	NULL	0	NULL	Crry ( - / - ) mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Complement activity and C3 levels in Crry ( - / - ) mice were markedly reduced .
	manualset3
249338	1	425513	7	NULL	NULL	0	NULL	Complementarity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Complementarity of hydrophobic properties in ATP-protein binding : a new criterion to rank docking solutions .
	manualset3
249339	2	425513	7	NULL	NULL	0	NULL	 hydrophobic properties	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Complementarity of hydrophobic properties in ATP-protein binding : a new criterion to rank docking solutions .
	manualset3
249340	3	425513	7	NULL	NULL	0	NULL	ATP-protein binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Complementarity of hydrophobic properties in ATP-protein binding : a new criterion to rank docking solutions .
	manualset3
249341	4	425513	7	NULL	NULL	0	NULL	new criterion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Complementarity of hydrophobic properties in ATP-protein binding : a new criterion to rank docking solutions .
	manualset3
249342	5	425513	7	NULL	NULL	0	NULL	docking solutions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Complementarity of hydrophobic properties in ATP-protein binding : a new criterion to rank docking solutions .
	manualset3
249343	1	425514	7	NULL	NULL	0	NULL	Complete amino acid sequence	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete amino acid sequence of plastocyanin from a green alga , Enteromorpha prolifera .
	manualset3
249344	2	425514	7	NULL	NULL	0	NULL	plastocyanin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete amino acid sequence of plastocyanin from a green alga , Enteromorpha prolifera .
	manualset3
249345	3	425514	7	NULL	NULL	0	NULL	green alga	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete amino acid sequence of plastocyanin from a green alga , Enteromorpha prolifera .
	manualset3
249346	4	425514	7	NULL	NULL	0	NULL	Enteromorpha prolifera	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete amino acid sequence of plastocyanin from a green alga , Enteromorpha prolifera .
	manualset3
249350	1	425515	7	NULL	NULL	0	NULL	Complete exchange	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete exchange occurred in the incubation at 0 degrees C between ( 3H ) progesterone and unlabelled progesterone and the saturable binding sites and the reaction attained apparent equilibrium within 2 h at this temperature .
	manualset3
249351	2	425515	7	NULL	NULL	0	NULL	incubation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete exchange occurred in the incubation at 0 degrees C between ( 3H ) progesterone and unlabelled progesterone and the saturable binding sites and the reaction attained apparent equilibrium within 2 h at this temperature .
	manualset3
249353	3	425515	7	NULL	NULL	0	NULL	 0 degrees C	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete exchange occurred in the incubation at 0 degrees C between ( 3H ) progesterone and unlabelled progesterone and the saturable binding sites and the reaction attained apparent equilibrium within 2 h at this temperature .
	manualset3
249354	4	425515	7	NULL	NULL	0	NULL	( 3H ) progesterone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete exchange occurred in the incubation at 0 degrees C between ( 3H ) progesterone and unlabelled progesterone and the saturable binding sites and the reaction attained apparent equilibrium within 2 h at this temperature .
	manualset3
249355	5	425515	7	NULL	NULL	0	NULL	unlabelled progesterone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete exchange occurred in the incubation at 0 degrees C between ( 3H ) progesterone and unlabelled progesterone and the saturable binding sites and the reaction attained apparent equilibrium within 2 h at this temperature .
	manualset3
249357	6	425515	7	NULL	NULL	0	NULL	saturable binding sites	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete exchange occurred in the incubation at 0 degrees C between ( 3H ) progesterone and unlabelled progesterone and the saturable binding sites and the reaction attained apparent equilibrium within 2 h at this temperature .
	manualset3
249358	7	425515	7	NULL	NULL	0	NULL	 reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete exchange occurred in the incubation at 0 degrees C between ( 3H ) progesterone and unlabelled progesterone and the saturable binding sites and the reaction attained apparent equilibrium within 2 h at this temperature .
	manualset3
249359	8	425515	7	NULL	NULL	0	NULL	equilibrium 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete exchange occurred in the incubation at 0 degrees C between ( 3H ) progesterone and unlabelled progesterone and the saturable binding sites and the reaction attained apparent equilibrium within 2 h at this temperature .
	manualset3
249360	9	425515	7	NULL	NULL	0	NULL	 2 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete exchange occurred in the incubation at 0 degrees C between ( 3H ) progesterone and unlabelled progesterone and the saturable binding sites and the reaction attained apparent equilibrium within 2 h at this temperature .
	manualset3
249361	10	425515	7	NULL	NULL	0	NULL	temperature	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete exchange occurred in the incubation at 0 degrees C between ( 3H ) progesterone and unlabelled progesterone and the saturable binding sites and the reaction attained apparent equilibrium within 2 h at this temperature .
	manualset3
249362	1	425516	7	NULL	NULL	0	NULL	 iron binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete iron binding with apotransferrin would apparently require very high apotransferrin doses .
	manualset3
249363	2	425516	7	NULL	NULL	0	NULL	apotransferrin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete iron binding with apotransferrin would apparently require very high apotransferrin doses .
	manualset3
249364	3	425516	7	NULL	NULL	0	NULL	high apotransferrin doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete iron binding with apotransferrin would apparently require very high apotransferrin doses .
	manualset3
249365	1	425517	7	NULL	NULL	0	NULL	strong inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete or strong inhibition of viral replication was observed when the patients ' PBMC were cultured with a high concentration of KD-247 .
	manualset3
249366	2	425517	7	NULL	NULL	0	NULL	viral replication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete or strong inhibition of viral replication was observed when the patients ' PBMC were cultured with a high concentration of KD-247 .
	manualset3
249367	3	425517	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete or strong inhibition of viral replication was observed when the patients ' PBMC were cultured with a high concentration of KD-247 .
	manualset3
249368	4	425517	7	NULL	NULL	0	NULL	PBMC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete or strong inhibition of viral replication was observed when the patients ' PBMC were cultured with a high concentration of KD-247 .
	manualset3
249369	5	425517	7	NULL	NULL	0	NULL	high concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete or strong inhibition of viral replication was observed when the patients ' PBMC were cultured with a high concentration of KD-247 .
	manualset3
249370	6	425517	7	NULL	NULL	0	NULL	KD-247	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete or strong inhibition of viral replication was observed when the patients ' PBMC were cultured with a high concentration of KD-247 .
	manualset3
249371	7	425517	7	NULL	NULL	0	NULL	Complete inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete or strong inhibition of viral replication was observed when the patients ' PBMC were cultured with a high concentration of KD-247 .
	manualset3
249373	1	425518	7	NULL	NULL	0	NULL	Complete recovery	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete recovery of metabolites during fermentations of clostridial cluster XIVa butyrate-producing colon bacteria allowed stoichiometric balancing of the metabolic pathway for butyrate production , including H2 formation .
	manualset3
249374	2	425518	7	NULL	NULL	0	NULL	metabolites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete recovery of metabolites during fermentations of clostridial cluster XIVa butyrate-producing colon bacteria allowed stoichiometric balancing of the metabolic pathway for butyrate production , including H2 formation .
	manualset3
249375	3	425518	7	NULL	NULL	0	NULL	fermentations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete recovery of metabolites during fermentations of clostridial cluster XIVa butyrate-producing colon bacteria allowed stoichiometric balancing of the metabolic pathway for butyrate production , including H2 formation .
	manualset3
249376	4	425518	7	NULL	NULL	0	NULL	clostridial cluster XIVa butyrate-producing colon bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete recovery of metabolites during fermentations of clostridial cluster XIVa butyrate-producing colon bacteria allowed stoichiometric balancing of the metabolic pathway for butyrate production , including H2 formation .
	manualset3
249377	5	425518	7	NULL	NULL	0	NULL	stoichiometric balancing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete recovery of metabolites during fermentations of clostridial cluster XIVa butyrate-producing colon bacteria allowed stoichiometric balancing of the metabolic pathway for butyrate production , including H2 formation .
	manualset3
249378	6	425518	7	NULL	NULL	0	NULL	metabolic pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete recovery of metabolites during fermentations of clostridial cluster XIVa butyrate-producing colon bacteria allowed stoichiometric balancing of the metabolic pathway for butyrate production , including H2 formation .
	manualset3
249380	7	425518	7	NULL	NULL	0	NULL	butyrate production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete recovery of metabolites during fermentations of clostridial cluster XIVa butyrate-producing colon bacteria allowed stoichiometric balancing of the metabolic pathway for butyrate production , including H2 formation .
	manualset3
249381	8	425518	7	NULL	NULL	0	NULL	H2 formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete recovery of metabolites during fermentations of clostridial cluster XIVa butyrate-producing colon bacteria allowed stoichiometric balancing of the metabolic pathway for butyrate production , including H2 formation .
	manualset3
249383	1	425519	7	NULL	NULL	0	NULL	Complete surgical resection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete surgical resection is the most effective curative treatment for lung cancer .
	manualset3
249385	2	425519	7	NULL	NULL	0	NULL	curative treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete surgical resection is the most effective curative treatment for lung cancer .
	manualset3
249386	3	425519	7	NULL	NULL	0	NULL	 lung cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete surgical resection is the most effective curative treatment for lung cancer .
	manualset3
249388	1	425520	7	NULL	NULL	0	NULL	Complete transcriptome 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete transcriptome and reporter fusion assay data revealed that MsmR positively regulates FCT region genes including Nra and cytolysin-mediated translocation system genes .
	manualset3
249389	2	425520	7	NULL	NULL	0	NULL	reporter fusion assay data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete transcriptome and reporter fusion assay data revealed that MsmR positively regulates FCT region genes including Nra and cytolysin-mediated translocation system genes .
	manualset3
249390	3	425520	7	NULL	NULL	0	NULL	MsmR 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete transcriptome and reporter fusion assay data revealed that MsmR positively regulates FCT region genes including Nra and cytolysin-mediated translocation system genes .
	manualset3
249391	4	425520	7	NULL	NULL	0	NULL	FCT region genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete transcriptome and reporter fusion assay data revealed that MsmR positively regulates FCT region genes including Nra and cytolysin-mediated translocation system genes .
	manualset3
249392	5	425520	7	NULL	NULL	0	NULL	Nra	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete transcriptome and reporter fusion assay data revealed that MsmR positively regulates FCT region genes including Nra and cytolysin-mediated translocation system genes .
	manualset3
249393	6	425520	7	NULL	NULL	0	NULL	cytolysin-mediated translocation system genes 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete transcriptome and reporter fusion assay data revealed that MsmR positively regulates FCT region genes including Nra and cytolysin-mediated translocation system genes .
	manualset3
249394	1	425521	7	NULL	NULL	0	NULL	Complete transection 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete transection of the common bile duct due to blunt ranuma .
	manualset3
249395	2	425521	7	NULL	NULL	0	NULL	common bile duct	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete transection of the common bile duct due to blunt ranuma .
	manualset3
249396	3	425521	7	NULL	NULL	0	NULL	 blunt ranuma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Complete transection of the common bile duct due to blunt ranuma .
	manualset3
249398	1	425522	7	NULL	NULL	0	NULL	Complex patterns	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Complex patterns of ADAM12 mRNA and protein splice variants in the human placenta .
	manualset3
249399	2	425522	7	NULL	NULL	0	NULL	ADAM12 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Complex patterns of ADAM12 mRNA and protein splice variants in the human placenta .
	manualset3
249400	3	425522	7	NULL	NULL	0	NULL	 protein splice variants	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Complex patterns of ADAM12 mRNA and protein splice variants in the human placenta .
	manualset3
249401	4	425522	7	NULL	NULL	0	NULL	human placenta	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Complex patterns of ADAM12 mRNA and protein splice variants in the human placenta .
	manualset3
249403	1	425523	7	NULL	NULL	NULL	NULL	Complex seizure characteristics	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Complex seizure characteristics are unlikely to help in discriminating phenotype subgroups for genetic studies of febrile seizures .
	manualset3
249404	2	425523	7	NULL	NULL	NULL	NULL	phenotype subgroups	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Complex seizure characteristics are unlikely to help in discriminating phenotype subgroups for genetic studies of febrile seizures .
	manualset3
249405	3	425523	7	NULL	NULL	0	NULL	genetic studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Complex seizure characteristics are unlikely to help in discriminating phenotype subgroups for genetic studies of febrile seizures .
	manualset3
249406	4	425523	7	NULL	NULL	0	NULL	febrile seizures	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Complex seizure characteristics are unlikely to help in discriminating phenotype subgroups for genetic studies of febrile seizures .
	manualset3
251596	5	425523	7	NULL	NULL	0	NULL	discriminating	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Complex seizure characteristics are unlikely to help in discriminating phenotype subgroups for genetic studies of febrile seizures .
	manualset3
249407	1	425524	7	NULL	NULL	NULL	NULL	Complex formation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Complex formation is influenced by post-translational protein modifications that arise from the cellular state or the DNA damage response , providing an increase in specificity and efficiency to the BER pathway .
	manualset3
249409	2	425524	7	NULL	NULL	0	NULL	 post-translational protein modifications	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Complex formation is influenced by post-translational protein modifications that arise from the cellular state or the DNA damage response , providing an increase in specificity and efficiency to the BER pathway .
	manualset3
249410	3	425524	7	NULL	NULL	0	NULL	cellular state	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Complex formation is influenced by post-translational protein modifications that arise from the cellular state or the DNA damage response , providing an increase in specificity and efficiency to the BER pathway .
	manualset3
249412	4	425524	7	NULL	NULL	0	NULL	DNA damage response	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Complex formation is influenced by post-translational protein modifications that arise from the cellular state or the DNA damage response , providing an increase in specificity and efficiency to the BER pathway .
	manualset3
249413	5	425524	7	NULL	NULL	0	NULL	specificity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Complex formation is influenced by post-translational protein modifications that arise from the cellular state or the DNA damage response , providing an increase in specificity and efficiency to the BER pathway .
	manualset3
249414	6	425524	7	NULL	NULL	0	NULL	efficiency 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Complex formation is influenced by post-translational protein modifications that arise from the cellular state or the DNA damage response , providing an increase in specificity and efficiency to the BER pathway .
	manualset3
249415	7	425524	7	NULL	NULL	0	NULL	BER pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Complex formation is influenced by post-translational protein modifications that arise from the cellular state or the DNA damage response , providing an increase in specificity and efficiency to the BER pathway .
	manualset3
249417	1	425525	7	NULL	NULL	0	NULL	Complex 1 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Complex 1 undergoes tert-butyl/arylamine exchange reactions to form 2 , 3 , ( Ti ( N-4-C ( 6 ) H ( 4 ) Me ) ( Me ( 2 ) calix ) ) ( 14 ) , ( Ti ( N-4-C ( 6 ) H ( 4 ) Fc ) ( Me ( 2 ) calix ) ) ( 15 ) ( Fc = Fe ( eta ( 5 ) - C ( 5 ) H ( 5 ) ) ( eta ( 5 ) - C ( 5 ) H ( 4 ) ) ) , and ( ( Ti ( Me ( 2 ) calix ) ) ( 2 ) ( mu - ( N-4-C ( 6 ) H ( 4 ) ) ( 2 ) CH ( 2 ) ) ) ( 16 ) .
	manualset3
249419	2	425525	7	NULL	NULL	0	NULL	tert-butyl/arylamine exchange reactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Complex 1 undergoes tert-butyl/arylamine exchange reactions to form 2 , 3 , ( Ti ( N-4-C ( 6 ) H ( 4 ) Me ) ( Me ( 2 ) calix ) ) ( 14 ) , ( Ti ( N-4-C ( 6 ) H ( 4 ) Fc ) ( Me ( 2 ) calix ) ) ( 15 ) ( Fc = Fe ( eta ( 5 ) - C ( 5 ) H ( 5 ) ) ( eta ( 5 ) - C ( 5 ) H ( 4 ) ) ) , and ( ( Ti ( Me ( 2 ) calix ) ) ( 2 ) ( mu - ( N-4-C ( 6 ) H ( 4 ) ) ( 2 ) CH ( 2 ) ) ) ( 16 ) .
	manualset3
249420	3	425525	7	NULL	NULL	0	NULL	2 , 3 , ( Ti ( N-4-C ( 6 ) H ( 4 ) Me ) ( Me ( 2 ) calix ) ) ( 14 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Complex 1 undergoes tert-butyl/arylamine exchange reactions to form 2 , 3 , ( Ti ( N-4-C ( 6 ) H ( 4 ) Me ) ( Me ( 2 ) calix ) ) ( 14 ) , ( Ti ( N-4-C ( 6 ) H ( 4 ) Fc ) ( Me ( 2 ) calix ) ) ( 15 ) ( Fc = Fe ( eta ( 5 ) - C ( 5 ) H ( 5 ) ) ( eta ( 5 ) - C ( 5 ) H ( 4 ) ) ) , and ( ( Ti ( Me ( 2 ) calix ) ) ( 2 ) ( mu - ( N-4-C ( 6 ) H ( 4 ) ) ( 2 ) CH ( 2 ) ) ) ( 16 ) .
	manualset3
249421	4	425525	7	NULL	NULL	0	NULL	 ( Ti ( N-4-C ( 6 ) H ( 4 ) Fc ) ( Me ( 2 ) calix ) ) ( 15 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Complex 1 undergoes tert-butyl/arylamine exchange reactions to form 2 , 3 , ( Ti ( N-4-C ( 6 ) H ( 4 ) Me ) ( Me ( 2 ) calix ) ) ( 14 ) , ( Ti ( N-4-C ( 6 ) H ( 4 ) Fc ) ( Me ( 2 ) calix ) ) ( 15 ) ( Fc = Fe ( eta ( 5 ) - C ( 5 ) H ( 5 ) ) ( eta ( 5 ) - C ( 5 ) H ( 4 ) ) ) , and ( ( Ti ( Me ( 2 ) calix ) ) ( 2 ) ( mu - ( N-4-C ( 6 ) H ( 4 ) ) ( 2 ) CH ( 2 ) ) ) ( 16 ) .
	manualset3
249422	5	425525	7	NULL	NULL	0	NULL	( Fc = Fe ( eta ( 5 ) - C ( 5 ) H ( 5 ) ) ( eta ( 5 ) - C ( 5 ) H ( 4 ) ) )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Complex 1 undergoes tert-butyl/arylamine exchange reactions to form 2 , 3 , ( Ti ( N-4-C ( 6 ) H ( 4 ) Me ) ( Me ( 2 ) calix ) ) ( 14 ) , ( Ti ( N-4-C ( 6 ) H ( 4 ) Fc ) ( Me ( 2 ) calix ) ) ( 15 ) ( Fc = Fe ( eta ( 5 ) - C ( 5 ) H ( 5 ) ) ( eta ( 5 ) - C ( 5 ) H ( 4 ) ) ) , and ( ( Ti ( Me ( 2 ) calix ) ) ( 2 ) ( mu - ( N-4-C ( 6 ) H ( 4 ) ) ( 2 ) CH ( 2 ) ) ) ( 16 ) .
	manualset3
249423	6	425525	7	NULL	NULL	0	NULL	( ( Ti ( Me ( 2 ) calix ) ) ( 2 ) ( mu - ( N-4-C ( 6 ) H ( 4 ) ) ( 2 ) CH ( 2 ) ) ) ( 16 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Complex 1 undergoes tert-butyl/arylamine exchange reactions to form 2 , 3 , ( Ti ( N-4-C ( 6 ) H ( 4 ) Me ) ( Me ( 2 ) calix ) ) ( 14 ) , ( Ti ( N-4-C ( 6 ) H ( 4 ) Fc ) ( Me ( 2 ) calix ) ) ( 15 ) ( Fc = Fe ( eta ( 5 ) - C ( 5 ) H ( 5 ) ) ( eta ( 5 ) - C ( 5 ) H ( 4 ) ) ) , and ( ( Ti ( Me ( 2 ) calix ) ) ( 2 ) ( mu - ( N-4-C ( 6 ) H ( 4 ) ) ( 2 ) CH ( 2 ) ) ) ( 16 ) .
	manualset3
249424	1	425526	7	NULL	NULL	0	NULL	Complexes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Complexes formed between thrombin and alpha 2-macroglobulin ( alpha 2M ) were studied by polyacrylamide gel electrophoresis .
	manualset3
249425	2	425526	7	NULL	NULL	0	NULL	thrombin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Complexes formed between thrombin and alpha 2-macroglobulin ( alpha 2M ) were studied by polyacrylamide gel electrophoresis .
	manualset3
249426	3	425526	7	NULL	NULL	0	NULL	alpha 2-macroglobulin ( alpha 2M )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Complexes formed between thrombin and alpha 2-macroglobulin ( alpha 2M ) were studied by polyacrylamide gel electrophoresis .
	manualset3
249427	4	425526	7	NULL	NULL	0	NULL	polyacrylamide gel electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Complexes formed between thrombin and alpha 2-macroglobulin ( alpha 2M ) were studied by polyacrylamide gel electrophoresis .
	manualset3
249428	1	425527	7	NULL	NULL	0	NULL	Complexes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Complexes of the enzyme with phospholipids were prepared using a method employing sodium dodecyl sulfate as a protein-solubilizing agent .
	manualset3
249429	2	425527	7	NULL	NULL	0	NULL	enzyme	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Complexes of the enzyme with phospholipids were prepared using a method employing sodium dodecyl sulfate as a protein-solubilizing agent .
	manualset3
249430	3	425527	7	NULL	NULL	0	NULL	 phospholipids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Complexes of the enzyme with phospholipids were prepared using a method employing sodium dodecyl sulfate as a protein-solubilizing agent .
	manualset3
249431	4	425527	7	NULL	NULL	0	NULL	method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Complexes of the enzyme with phospholipids were prepared using a method employing sodium dodecyl sulfate as a protein-solubilizing agent .
	manualset3
249432	5	425527	7	NULL	NULL	0	NULL	sodium dodecyl sulfate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Complexes of the enzyme with phospholipids were prepared using a method employing sodium dodecyl sulfate as a protein-solubilizing agent .
	manualset3
249433	6	425527	7	NULL	NULL	0	NULL	protein-solubilizing agent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Complexes of the enzyme with phospholipids were prepared using a method employing sodium dodecyl sulfate as a protein-solubilizing agent .
	manualset3
249434	1	425528	7	NULL	NULL	0	NULL	Compliance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compliance with science : consent or coercion in newborn screening .
	manualset3
249435	2	425528	7	NULL	NULL	0	NULL	science	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Compliance with science : consent or coercion in newborn screening .
	manualset3
249436	3	425528	7	NULL	NULL	0	NULL	consent	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compliance with science : consent or coercion in newborn screening .
	manualset3
249437	4	425528	7	NULL	NULL	0	NULL	coercion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compliance with science : consent or coercion in newborn screening .
	manualset3
249438	5	425528	7	NULL	NULL	0	NULL	newborn screening	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Compliance with science : consent or coercion in newborn screening .
	manualset3
249439	1	425529	7	NULL	NULL	0	NULL	Complications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Complications associated with bone cementing for the treatment of giant cell tumors of bone .
	manualset3
249440	2	425529	7	NULL	NULL	0	NULL	bone cementing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Complications associated with bone cementing for the treatment of giant cell tumors of bone .
	manualset3
249441	3	425529	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Complications associated with bone cementing for the treatment of giant cell tumors of bone .
	manualset3
249442	4	425529	7	NULL	NULL	0	NULL	giant cell tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Complications associated with bone cementing for the treatment of giant cell tumors of bone .
	manualset3
249443	5	425529	7	NULL	NULL	0	NULL	bone	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Complications associated with bone cementing for the treatment of giant cell tumors of bone .
	manualset3
249444	1	425530	7	NULL	NULL	0	NULL	Complications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Complications consisted of four episodes of otitis media caused by Staphylococcus aureus and one rejection episode that was treated on an outpatient basis with an intravenous methylprednisolone sodium succinate pulse .
	manualset3
249445	2	425530	7	NULL	NULL	0	NULL	four episodes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Complications consisted of four episodes of otitis media caused by Staphylococcus aureus and one rejection episode that was treated on an outpatient basis with an intravenous methylprednisolone sodium succinate pulse .
	manualset3
249446	3	425530	7	NULL	NULL	0	NULL	otitis media	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Complications consisted of four episodes of otitis media caused by Staphylococcus aureus and one rejection episode that was treated on an outpatient basis with an intravenous methylprednisolone sodium succinate pulse .
	manualset3
249447	4	425530	7	NULL	NULL	0	NULL	Staphylococcus aureus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Complications consisted of four episodes of otitis media caused by Staphylococcus aureus and one rejection episode that was treated on an outpatient basis with an intravenous methylprednisolone sodium succinate pulse .
	manualset3
249448	5	425530	7	NULL	NULL	0	NULL	one rejection episode	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Complications consisted of four episodes of otitis media caused by Staphylococcus aureus and one rejection episode that was treated on an outpatient basis with an intravenous methylprednisolone sodium succinate pulse .
	manualset3
249449	6	425530	7	NULL	NULL	0	NULL	outpatient basis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Complications consisted of four episodes of otitis media caused by Staphylococcus aureus and one rejection episode that was treated on an outpatient basis with an intravenous methylprednisolone sodium succinate pulse .
	manualset3
249450	7	425530	7	NULL	NULL	0	NULL	intravenous methylprednisolone sodium succinate pulse	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Complications consisted of four episodes of otitis media caused by Staphylococcus aureus and one rejection episode that was treated on an outpatient basis with an intravenous methylprednisolone sodium succinate pulse .
	manualset3
249451	1	425531	7	NULL	NULL	0	NULL	Jaffe-Campanacci syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Jaffe-Campanacci syndrome : report of a case ) .
	manualset3
249452	2	425531	7	NULL	NULL	0	NULL	report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Jaffe-Campanacci syndrome : report of a case ) .
	manualset3
249453	3	425531	7	NULL	NULL	0	NULL	case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Jaffe-Campanacci syndrome : report of a case ) .
	manualset3
249527	1	425532	7	NULL	NULL	0	NULL	Complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Complications of treatment can be divided into : failure to correct , recurrence and overcorrection .
	manualset3
249528	2	425532	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Complications of treatment can be divided into : failure to correct , recurrence and overcorrection .
	manualset3
249529	3	425532	7	NULL	NULL	0	NULL	failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Complications of treatment can be divided into : failure to correct , recurrence and overcorrection .
	manualset3
249530	4	425532	7	NULL	NULL	0	NULL	overcorrection 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Complications of treatment can be divided into : failure to correct , recurrence and overcorrection .
	manualset3
249531	1	425533	7	NULL	NULL	0	NULL	Complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Complications related to the ablation or injury of cranial nerves IX , X , XI , and XII are commonly seen .
	manualset3
249532	2	425533	7	NULL	NULL	0	NULL	ablation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Complications related to the ablation or injury of cranial nerves IX , X , XI , and XII are commonly seen .
	manualset3
249533	3	425533	7	NULL	NULL	0	NULL	injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Complications related to the ablation or injury of cranial nerves IX , X , XI , and XII are commonly seen .
	manualset3
249534	4	425533	7	NULL	NULL	NULL	NULL	 cranial nerves IX	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Complications related to the ablation or injury of cranial nerves IX , X , XI , and XII are commonly seen .
	manualset3
249535	5	425533	7	NULL	NULL	0	NULL	cranial nerves X	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Complications related to the ablation or injury of cranial nerves IX , X , XI , and XII are commonly seen .
	manualset3
249536	6	425533	7	NULL	NULL	0	NULL	cranial nerves XI	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Complications related to the ablation or injury of cranial nerves IX , X , XI , and XII are commonly seen .
	manualset3
249537	7	425533	7	NULL	NULL	0	NULL	cranial nerves XII 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Complications related to the ablation or injury of cranial nerves IX , X , XI , and XII are commonly seen .
	manualset3
249538	1	425534	7	NULL	NULL	0	NULL	Composite films 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Composite films of nanosized TiO2 particles , which contained rutile as the only detected crystal modification , and poly ( vinyl alcohol ) , poly ( vinyl pyrrolidone ) or poly ( 4-vinylpyridine ) were prepared from aqueous dispersions .
	manualset3
249539	2	425534	7	NULL	NULL	0	NULL	nanosized TiO2 particles	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Composite films of nanosized TiO2 particles , which contained rutile as the only detected crystal modification , and poly ( vinyl alcohol ) , poly ( vinyl pyrrolidone ) or poly ( 4-vinylpyridine ) were prepared from aqueous dispersions .
	manualset3
249540	3	425534	7	NULL	NULL	0	NULL	crystal modification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Composite films of nanosized TiO2 particles , which contained rutile as the only detected crystal modification , and poly ( vinyl alcohol ) , poly ( vinyl pyrrolidone ) or poly ( 4-vinylpyridine ) were prepared from aqueous dispersions .
	manualset3
249541	4	425534	7	NULL	NULL	0	NULL	poly ( vinyl alcohol )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Composite films of nanosized TiO2 particles , which contained rutile as the only detected crystal modification , and poly ( vinyl alcohol ) , poly ( vinyl pyrrolidone ) or poly ( 4-vinylpyridine ) were prepared from aqueous dispersions .
	manualset3
249542	5	425534	7	NULL	NULL	0	NULL	poly ( vinyl pyrrolidone )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Composite films of nanosized TiO2 particles , which contained rutile as the only detected crystal modification , and poly ( vinyl alcohol ) , poly ( vinyl pyrrolidone ) or poly ( 4-vinylpyridine ) were prepared from aqueous dispersions .
	manualset3
249543	6	425534	7	NULL	NULL	0	NULL	 poly ( 4-vinylpyridine ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Composite films of nanosized TiO2 particles , which contained rutile as the only detected crystal modification , and poly ( vinyl alcohol ) , poly ( vinyl pyrrolidone ) or poly ( 4-vinylpyridine ) were prepared from aqueous dispersions .
	manualset3
249544	7	425534	7	NULL	NULL	0	NULL	 aqueous dispersions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Composite films of nanosized TiO2 particles , which contained rutile as the only detected crystal modification , and poly ( vinyl alcohol ) , poly ( vinyl pyrrolidone ) or poly ( 4-vinylpyridine ) were prepared from aqueous dispersions .
	manualset3
249545	1	425535	7	NULL	NULL	0	NULL	Composition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Composition of the zooplankton community , with emphasis in copepods , in Punta Morales , Golfo De Nicoya , Costa Rica .
	manualset3
249546	2	425535	7	NULL	NULL	0	NULL	zooplankton community	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Composition of the zooplankton community , with emphasis in copepods , in Punta Morales , Golfo De Nicoya , Costa Rica .
	manualset3
249547	3	425535	7	NULL	NULL	0	NULL	copepods	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Composition of the zooplankton community , with emphasis in copepods , in Punta Morales , Golfo De Nicoya , Costa Rica .
	manualset3
249548	4	425535	7	NULL	NULL	0	NULL	Punta Morales	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Composition of the zooplankton community , with emphasis in copepods , in Punta Morales , Golfo De Nicoya , Costa Rica .
	manualset3
249549	5	425535	7	NULL	NULL	0	NULL	Golfo De Nicoya 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Composition of the zooplankton community , with emphasis in copepods , in Punta Morales , Golfo De Nicoya , Costa Rica .
	manualset3
249550	6	425535	7	NULL	NULL	0	NULL	Costa Rica	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Composition of the zooplankton community , with emphasis in copepods , in Punta Morales , Golfo De Nicoya , Costa Rica .
	manualset3
249551	1	425536	7	NULL	NULL	0	NULL	Compound 14 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 14 , the first example in this series , was found to be a potent FPT inhibitor ( I50 = 60 nM ) .
	manualset3
249552	2	425536	7	NULL	NULL	0	NULL	 first example	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 14 , the first example in this series , was found to be a potent FPT inhibitor ( I50 = 60 nM ) .
	manualset3
249553	3	425536	7	NULL	NULL	0	NULL	series	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 14 , the first example in this series , was found to be a potent FPT inhibitor ( I50 = 60 nM ) .
	manualset3
249554	4	425536	7	NULL	NULL	0	NULL	potent FPT inhibitor 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 14 , the first example in this series , was found to be a potent FPT inhibitor ( I50 = 60 nM ) .
	manualset3
249555	5	425536	7	NULL	NULL	0	NULL	I50 = 60 nM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 14 , the first example in this series , was found to be a potent FPT inhibitor ( I50 = 60 nM ) .
	manualset3
249556	1	425537	7	NULL	NULL	NULL	NULL	Compound 2 ( 6 , 7-dichloro-2-methylsulfonyl-2-N-tert-butylaminoquinoxaline )	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Compound 2 ( 6 , 7-dichloro-2-methylsulfonyl-2-N-tert-butylaminoquinoxaline ) and compound B ( 4 - ( 3 - ( benzyloxy ) phenyl ) -2 - ( ethylsulfinyl ) -6 - ( trifluoromethyl ) pyrimidine ) have been described as small molecule , ago-allosteric modulators of GLP-1R .
	manualset3
249557	2	425537	7	NULL	NULL	0	NULL	compound B ( 4 - ( 3 - ( benzyloxy ) phenyl ) -2 - ( ethylsulfinyl ) -6 - ( trifluoromethyl ) pyrimidine )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 2 ( 6 , 7-dichloro-2-methylsulfonyl-2-N-tert-butylaminoquinoxaline ) and compound B ( 4 - ( 3 - ( benzyloxy ) phenyl ) -2 - ( ethylsulfinyl ) -6 - ( trifluoromethyl ) pyrimidine ) have been described as small molecule , ago-allosteric modulators of GLP-1R .
	manualset3
249558	3	425537	7	NULL	NULL	0	NULL	small molecule	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 2 ( 6 , 7-dichloro-2-methylsulfonyl-2-N-tert-butylaminoquinoxaline ) and compound B ( 4 - ( 3 - ( benzyloxy ) phenyl ) -2 - ( ethylsulfinyl ) -6 - ( trifluoromethyl ) pyrimidine ) have been described as small molecule , ago-allosteric modulators of GLP-1R .
	manualset3
249560	4	425537	7	NULL	NULL	0	NULL	ago-allosteric modulators	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 2 ( 6 , 7-dichloro-2-methylsulfonyl-2-N-tert-butylaminoquinoxaline ) and compound B ( 4 - ( 3 - ( benzyloxy ) phenyl ) -2 - ( ethylsulfinyl ) -6 - ( trifluoromethyl ) pyrimidine ) have been described as small molecule , ago-allosteric modulators of GLP-1R .
	manualset3
249561	5	425537	7	NULL	NULL	0	NULL	GLP-1R	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 2 ( 6 , 7-dichloro-2-methylsulfonyl-2-N-tert-butylaminoquinoxaline ) and compound B ( 4 - ( 3 - ( benzyloxy ) phenyl ) -2 - ( ethylsulfinyl ) -6 - ( trifluoromethyl ) pyrimidine ) have been described as small molecule , ago-allosteric modulators of GLP-1R .
	manualset3
249563	1	425538	7	NULL	NULL	0	NULL	Compound 2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 2 produced 100 % , 43 % , and 37 % reduction of viral replication at 50 , 10 , and 2microg/mL concentrations , respectively .
	manualset3
249564	2	425538	7	NULL	NULL	0	NULL	 100 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 2 produced 100 % , 43 % , and 37 % reduction of viral replication at 50 , 10 , and 2microg/mL concentrations , respectively .
	manualset3
249565	3	425538	7	NULL	NULL	0	NULL	43 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 2 produced 100 % , 43 % , and 37 % reduction of viral replication at 50 , 10 , and 2microg/mL concentrations , respectively .
	manualset3
249566	4	425538	7	NULL	NULL	0	NULL	 37 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 2 produced 100 % , 43 % , and 37 % reduction of viral replication at 50 , 10 , and 2microg/mL concentrations , respectively .
	manualset3
249567	5	425538	7	NULL	NULL	0	NULL	reduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 2 produced 100 % , 43 % , and 37 % reduction of viral replication at 50 , 10 , and 2microg/mL concentrations , respectively .
	manualset3
249568	6	425538	7	NULL	NULL	0	NULL	 viral replication	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 2 produced 100 % , 43 % , and 37 % reduction of viral replication at 50 , 10 , and 2microg/mL concentrations , respectively .
	manualset3
249569	7	425538	7	NULL	NULL	0	NULL	50 microg/mL	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 2 produced 100 % , 43 % , and 37 % reduction of viral replication at 50 , 10 , and 2microg/mL concentrations , respectively .
	manualset3
249570	8	425538	7	NULL	NULL	0	NULL	10 microg/mL	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 2 produced 100 % , 43 % , and 37 % reduction of viral replication at 50 , 10 , and 2microg/mL concentrations , respectively .
	manualset3
249571	9	425538	7	NULL	NULL	0	NULL	2microg/mL	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 2 produced 100 % , 43 % , and 37 % reduction of viral replication at 50 , 10 , and 2microg/mL concentrations , respectively .
	manualset3
249572	10	425538	7	NULL	NULL	0	NULL	concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 2 produced 100 % , 43 % , and 37 % reduction of viral replication at 50 , 10 , and 2microg/mL concentrations , respectively .
	manualset3
249573	1	425539	7	NULL	NULL	0	NULL	Compound 3a	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 3a was more potent than 3b against tumor cells .
	manualset3
249574	2	425539	7	NULL	NULL	0	NULL	Compound 3b	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 3a was more potent than 3b against tumor cells .
	manualset3
249575	3	425539	7	NULL	NULL	0	NULL	tumor cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 3a was more potent than 3b against tumor cells .
	manualset3
249576	1	425540	7	NULL	NULL	0	NULL	Japanese methods	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Japanese methods of psychotherapy and their socio-cultural determinants .
	manualset3
249577	2	425540	7	NULL	NULL	0	NULL	psychotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Japanese methods of psychotherapy and their socio-cultural determinants .
	manualset3
249578	3	425540	7	NULL	NULL	0	NULL	socio-cultural determinants	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Japanese methods of psychotherapy and their socio-cultural determinants .
	manualset3
249582	1	425541	7	NULL	NULL	0	NULL	Compound 4	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 4 has a three-dimensional triply-interpenetrated diamondoid structure , with dimethylammonium cations and DMF molecules included within the pores .
	manualset3
249584	2	425541	7	NULL	NULL	0	NULL	 three-dimensional triply-interpenetrated diamondoid structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 4 has a three-dimensional triply-interpenetrated diamondoid structure , with dimethylammonium cations and DMF molecules included within the pores .
	manualset3
249585	3	425541	7	NULL	NULL	0	NULL	dimethylammonium cations	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 4 has a three-dimensional triply-interpenetrated diamondoid structure , with dimethylammonium cations and DMF molecules included within the pores .
	manualset3
249587	4	425541	7	NULL	NULL	0	NULL	DMF molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 4 has a three-dimensional triply-interpenetrated diamondoid structure , with dimethylammonium cations and DMF molecules included within the pores .
	manualset3
249588	5	425541	7	NULL	NULL	0	NULL	pores	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 4 has a three-dimensional triply-interpenetrated diamondoid structure , with dimethylammonium cations and DMF molecules included within the pores .
	manualset3
249870	1	425542	7	NULL	NULL	0	NULL	Compound 4	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 4 inhibited MAO-B with an IC ( 50 ) of 27 nM and MAO-A with an IC ( 50 ) of 2.3 M. Radiolabeling of precursor 3 and subsequent hydrolysis of the protecting group towards ( 1S , 2 S ) -2 - ( ( 18 ) F ) fluoro-N - ( prop-2-yn-1-yl ) indan-1-amine ( 6 ) was successfully accomplished with an radiochemical yield of 40-70 % , a radiochemical purity higher than 99 % and a specific radioactivity higher than 200GBq/mol .
	manualset3
249873	2	425542	7	NULL	NULL	0	NULL	MAO-B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 4 inhibited MAO-B with an IC ( 50 ) of 27 nM and MAO-A with an IC ( 50 ) of 2.3 M. Radiolabeling of precursor 3 and subsequent hydrolysis of the protecting group towards ( 1S , 2 S ) -2 - ( ( 18 ) F ) fluoro-N - ( prop-2-yn-1-yl ) indan-1-amine ( 6 ) was successfully accomplished with an radiochemical yield of 40-70 % , a radiochemical purity higher than 99 % and a specific radioactivity higher than 200GBq/mol .
	manualset3
249875	3	425542	7	NULL	NULL	0	NULL	IC ( 50 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 4 inhibited MAO-B with an IC ( 50 ) of 27 nM and MAO-A with an IC ( 50 ) of 2.3 M. Radiolabeling of precursor 3 and subsequent hydrolysis of the protecting group towards ( 1S , 2 S ) -2 - ( ( 18 ) F ) fluoro-N - ( prop-2-yn-1-yl ) indan-1-amine ( 6 ) was successfully accomplished with an radiochemical yield of 40-70 % , a radiochemical purity higher than 99 % and a specific radioactivity higher than 200GBq/mol .
	manualset3
249877	4	425542	7	NULL	NULL	0	NULL	27 nM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 4 inhibited MAO-B with an IC ( 50 ) of 27 nM and MAO-A with an IC ( 50 ) of 2.3 M. Radiolabeling of precursor 3 and subsequent hydrolysis of the protecting group towards ( 1S , 2 S ) -2 - ( ( 18 ) F ) fluoro-N - ( prop-2-yn-1-yl ) indan-1-amine ( 6 ) was successfully accomplished with an radiochemical yield of 40-70 % , a radiochemical purity higher than 99 % and a specific radioactivity higher than 200GBq/mol .
	manualset3
249878	5	425542	7	NULL	NULL	0	NULL	MAO-A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 4 inhibited MAO-B with an IC ( 50 ) of 27 nM and MAO-A with an IC ( 50 ) of 2.3 M. Radiolabeling of precursor 3 and subsequent hydrolysis of the protecting group towards ( 1S , 2 S ) -2 - ( ( 18 ) F ) fluoro-N - ( prop-2-yn-1-yl ) indan-1-amine ( 6 ) was successfully accomplished with an radiochemical yield of 40-70 % , a radiochemical purity higher than 99 % and a specific radioactivity higher than 200GBq/mol .
	manualset3
249879	6	425542	7	NULL	NULL	0	NULL	IC ( 50 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 4 inhibited MAO-B with an IC ( 50 ) of 27 nM and MAO-A with an IC ( 50 ) of 2.3 M. Radiolabeling of precursor 3 and subsequent hydrolysis of the protecting group towards ( 1S , 2 S ) -2 - ( ( 18 ) F ) fluoro-N - ( prop-2-yn-1-yl ) indan-1-amine ( 6 ) was successfully accomplished with an radiochemical yield of 40-70 % , a radiochemical purity higher than 99 % and a specific radioactivity higher than 200GBq/mol .
	manualset3
249881	7	425542	7	NULL	NULL	0	NULL	2.3 M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 4 inhibited MAO-B with an IC ( 50 ) of 27 nM and MAO-A with an IC ( 50 ) of 2.3 M. Radiolabeling of precursor 3 and subsequent hydrolysis of the protecting group towards ( 1S , 2 S ) -2 - ( ( 18 ) F ) fluoro-N - ( prop-2-yn-1-yl ) indan-1-amine ( 6 ) was successfully accomplished with an radiochemical yield of 40-70 % , a radiochemical purity higher than 99 % and a specific radioactivity higher than 200GBq/mol .
	manualset3
249882	8	425542	7	NULL	NULL	0	NULL	Radiolabeling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 4 inhibited MAO-B with an IC ( 50 ) of 27 nM and MAO-A with an IC ( 50 ) of 2.3 M. Radiolabeling of precursor 3 and subsequent hydrolysis of the protecting group towards ( 1S , 2 S ) -2 - ( ( 18 ) F ) fluoro-N - ( prop-2-yn-1-yl ) indan-1-amine ( 6 ) was successfully accomplished with an radiochemical yield of 40-70 % , a radiochemical purity higher than 99 % and a specific radioactivity higher than 200GBq/mol .
	manualset3
249883	9	425542	7	NULL	NULL	0	NULL	precursor 3	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 4 inhibited MAO-B with an IC ( 50 ) of 27 nM and MAO-A with an IC ( 50 ) of 2.3 M. Radiolabeling of precursor 3 and subsequent hydrolysis of the protecting group towards ( 1S , 2 S ) -2 - ( ( 18 ) F ) fluoro-N - ( prop-2-yn-1-yl ) indan-1-amine ( 6 ) was successfully accomplished with an radiochemical yield of 40-70 % , a radiochemical purity higher than 99 % and a specific radioactivity higher than 200GBq/mol .
	manualset3
249885	10	425542	7	NULL	NULL	0	NULL	hydrolysis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 4 inhibited MAO-B with an IC ( 50 ) of 27 nM and MAO-A with an IC ( 50 ) of 2.3 M. Radiolabeling of precursor 3 and subsequent hydrolysis of the protecting group towards ( 1S , 2 S ) -2 - ( ( 18 ) F ) fluoro-N - ( prop-2-yn-1-yl ) indan-1-amine ( 6 ) was successfully accomplished with an radiochemical yield of 40-70 % , a radiochemical purity higher than 99 % and a specific radioactivity higher than 200GBq/mol .
	manualset3
249887	11	425542	7	NULL	NULL	0	NULL	protecting group	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 4 inhibited MAO-B with an IC ( 50 ) of 27 nM and MAO-A with an IC ( 50 ) of 2.3 M. Radiolabeling of precursor 3 and subsequent hydrolysis of the protecting group towards ( 1S , 2 S ) -2 - ( ( 18 ) F ) fluoro-N - ( prop-2-yn-1-yl ) indan-1-amine ( 6 ) was successfully accomplished with an radiochemical yield of 40-70 % , a radiochemical purity higher than 99 % and a specific radioactivity higher than 200GBq/mol .
	manualset3
249888	12	425542	7	NULL	NULL	0	NULL	( 1S , 2 S ) -2 - ( ( 18 ) F ) fluoro-N - ( prop-2-yn-1-yl ) indan-1-amine ( 6 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 4 inhibited MAO-B with an IC ( 50 ) of 27 nM and MAO-A with an IC ( 50 ) of 2.3 M. Radiolabeling of precursor 3 and subsequent hydrolysis of the protecting group towards ( 1S , 2 S ) -2 - ( ( 18 ) F ) fluoro-N - ( prop-2-yn-1-yl ) indan-1-amine ( 6 ) was successfully accomplished with an radiochemical yield of 40-70 % , a radiochemical purity higher than 99 % and a specific radioactivity higher than 200GBq/mol .
	manualset3
249889	13	425542	7	NULL	NULL	0	NULL	 radiochemical yield	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 4 inhibited MAO-B with an IC ( 50 ) of 27 nM and MAO-A with an IC ( 50 ) of 2.3 M. Radiolabeling of precursor 3 and subsequent hydrolysis of the protecting group towards ( 1S , 2 S ) -2 - ( ( 18 ) F ) fluoro-N - ( prop-2-yn-1-yl ) indan-1-amine ( 6 ) was successfully accomplished with an radiochemical yield of 40-70 % , a radiochemical purity higher than 99 % and a specific radioactivity higher than 200GBq/mol .
	manualset3
249890	14	425542	7	NULL	NULL	0	NULL	40-70 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 4 inhibited MAO-B with an IC ( 50 ) of 27 nM and MAO-A with an IC ( 50 ) of 2.3 M. Radiolabeling of precursor 3 and subsequent hydrolysis of the protecting group towards ( 1S , 2 S ) -2 - ( ( 18 ) F ) fluoro-N - ( prop-2-yn-1-yl ) indan-1-amine ( 6 ) was successfully accomplished with an radiochemical yield of 40-70 % , a radiochemical purity higher than 99 % and a specific radioactivity higher than 200GBq/mol .
	manualset3
249891	15	425542	7	NULL	NULL	0	NULL	radiochemical purity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 4 inhibited MAO-B with an IC ( 50 ) of 27 nM and MAO-A with an IC ( 50 ) of 2.3 M. Radiolabeling of precursor 3 and subsequent hydrolysis of the protecting group towards ( 1S , 2 S ) -2 - ( ( 18 ) F ) fluoro-N - ( prop-2-yn-1-yl ) indan-1-amine ( 6 ) was successfully accomplished with an radiochemical yield of 40-70 % , a radiochemical purity higher than 99 % and a specific radioactivity higher than 200GBq/mol .
	manualset3
249892	16	425542	7	NULL	NULL	0	NULL	 99 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 4 inhibited MAO-B with an IC ( 50 ) of 27 nM and MAO-A with an IC ( 50 ) of 2.3 M. Radiolabeling of precursor 3 and subsequent hydrolysis of the protecting group towards ( 1S , 2 S ) -2 - ( ( 18 ) F ) fluoro-N - ( prop-2-yn-1-yl ) indan-1-amine ( 6 ) was successfully accomplished with an radiochemical yield of 40-70 % , a radiochemical purity higher than 99 % and a specific radioactivity higher than 200GBq/mol .
	manualset3
249893	17	425542	7	NULL	NULL	0	NULL	specific radioactivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 4 inhibited MAO-B with an IC ( 50 ) of 27 nM and MAO-A with an IC ( 50 ) of 2.3 M. Radiolabeling of precursor 3 and subsequent hydrolysis of the protecting group towards ( 1S , 2 S ) -2 - ( ( 18 ) F ) fluoro-N - ( prop-2-yn-1-yl ) indan-1-amine ( 6 ) was successfully accomplished with an radiochemical yield of 40-70 % , a radiochemical purity higher than 99 % and a specific radioactivity higher than 200GBq/mol .
	manualset3
249894	18	425542	7	NULL	NULL	0	NULL	200GBq/mol	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 4 inhibited MAO-B with an IC ( 50 ) of 27 nM and MAO-A with an IC ( 50 ) of 2.3 M. Radiolabeling of precursor 3 and subsequent hydrolysis of the protecting group towards ( 1S , 2 S ) -2 - ( ( 18 ) F ) fluoro-N - ( prop-2-yn-1-yl ) indan-1-amine ( 6 ) was successfully accomplished with an radiochemical yield of 40-70 % , a radiochemical purity higher than 99 % and a specific radioactivity higher than 200GBq/mol .
	manualset3
249895	1	425543	7	NULL	NULL	0	NULL	Compound 8b	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 8b was the most active with IC ( 50 ) of 0.0330.014 M. Generally , among the tested compounds , those containing a free carboxylic acid functional group on the pyrazole ring were the most active and this finding was supported by the docking results performed for the active compounds .
	manualset3
249897	2	425543	7	NULL	NULL	0	NULL	IC ( 50 ) 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 8b was the most active with IC ( 50 ) of 0.0330.014 M. Generally , among the tested compounds , those containing a free carboxylic acid functional group on the pyrazole ring were the most active and this finding was supported by the docking results performed for the active compounds .
	manualset3
249898	3	425543	7	NULL	NULL	0	NULL	 0.0330.014 M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 8b was the most active with IC ( 50 ) of 0.0330.014 M. Generally , among the tested compounds , those containing a free carboxylic acid functional group on the pyrazole ring were the most active and this finding was supported by the docking results performed for the active compounds .
	manualset3
249899	4	425543	7	NULL	NULL	0	NULL	tested compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 8b was the most active with IC ( 50 ) of 0.0330.014 M. Generally , among the tested compounds , those containing a free carboxylic acid functional group on the pyrazole ring were the most active and this finding was supported by the docking results performed for the active compounds .
	manualset3
249900	5	425543	7	NULL	NULL	0	NULL	free carboxylic acid functional group	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 8b was the most active with IC ( 50 ) of 0.0330.014 M. Generally , among the tested compounds , those containing a free carboxylic acid functional group on the pyrazole ring were the most active and this finding was supported by the docking results performed for the active compounds .
	manualset3
249901	6	425543	7	NULL	NULL	0	NULL	 pyrazole ring	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 8b was the most active with IC ( 50 ) of 0.0330.014 M. Generally , among the tested compounds , those containing a free carboxylic acid functional group on the pyrazole ring were the most active and this finding was supported by the docking results performed for the active compounds .
	manualset3
249902	7	425543	7	NULL	NULL	0	NULL	finding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 8b was the most active with IC ( 50 ) of 0.0330.014 M. Generally , among the tested compounds , those containing a free carboxylic acid functional group on the pyrazole ring were the most active and this finding was supported by the docking results performed for the active compounds .
	manualset3
249903	8	425543	7	NULL	NULL	0	NULL	docking results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 8b was the most active with IC ( 50 ) of 0.0330.014 M. Generally , among the tested compounds , those containing a free carboxylic acid functional group on the pyrazole ring were the most active and this finding was supported by the docking results performed for the active compounds .
	manualset3
249904	9	425543	7	NULL	NULL	0	NULL	active compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compound 8b was the most active with IC ( 50 ) of 0.0330.014 M. Generally , among the tested compounds , those containing a free carboxylic acid functional group on the pyrazole ring were the most active and this finding was supported by the docking results performed for the active compounds .
	manualset3
249919	1	425544	7	NULL	NULL	0	NULL	compression moulded materials	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounded and compression moulded materials were evaluated using various techniques including thermogravimatric analysis , scanning electron microscopy , differential scanning calorimetry and dynamic mechanical analysis .
	manualset3
249921	2	425544	7	NULL	NULL	0	NULL	techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounded and compression moulded materials were evaluated using various techniques including thermogravimatric analysis , scanning electron microscopy , differential scanning calorimetry and dynamic mechanical analysis .
	manualset3
249923	3	425544	7	NULL	NULL	0	NULL	thermogravimatric analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounded and compression moulded materials were evaluated using various techniques including thermogravimatric analysis , scanning electron microscopy , differential scanning calorimetry and dynamic mechanical analysis .
	manualset3
249925	4	425544	7	NULL	NULL	0	NULL	scanning electron microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounded and compression moulded materials were evaluated using various techniques including thermogravimatric analysis , scanning electron microscopy , differential scanning calorimetry and dynamic mechanical analysis .
	manualset3
249928	5	425544	7	NULL	NULL	0	NULL	differential scanning calorimetry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounded and compression moulded materials were evaluated using various techniques including thermogravimatric analysis , scanning electron microscopy , differential scanning calorimetry and dynamic mechanical analysis .
	manualset3
249930	6	425544	7	NULL	NULL	NULL	NULL	dynamic mechanical analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Compounded and compression moulded materials were evaluated using various techniques including thermogravimatric analysis , scanning electron microscopy , differential scanning calorimetry and dynamic mechanical analysis .
	manualset3
249942	1	425545	7	NULL	NULL	0	NULL	Compounded productivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounded productivity is the unique benefit of kaizen , and its principles are change , efficiency , performance of key essential steps , and the elimination of waste through small and continuous process improvements .
	manualset3
249944	2	425545	7	NULL	NULL	0	NULL	unique benefit	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounded productivity is the unique benefit of kaizen , and its principles are change , efficiency , performance of key essential steps , and the elimination of waste through small and continuous process improvements .
	manualset3
249947	3	425545	7	NULL	NULL	0	NULL	kaizen	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounded productivity is the unique benefit of kaizen , and its principles are change , efficiency , performance of key essential steps , and the elimination of waste through small and continuous process improvements .
	manualset3
249949	4	425545	7	NULL	NULL	0	NULL	 principles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounded productivity is the unique benefit of kaizen , and its principles are change , efficiency , performance of key essential steps , and the elimination of waste through small and continuous process improvements .
	manualset3
249951	5	425545	7	NULL	NULL	0	NULL	key essential steps	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounded productivity is the unique benefit of kaizen , and its principles are change , efficiency , performance of key essential steps , and the elimination of waste through small and continuous process improvements .
	manualset3
249953	6	425545	7	NULL	NULL	0	NULL	elimination 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounded productivity is the unique benefit of kaizen , and its principles are change , efficiency , performance of key essential steps , and the elimination of waste through small and continuous process improvements .
	manualset3
249955	7	425545	7	NULL	NULL	0	NULL	 waste	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounded productivity is the unique benefit of kaizen , and its principles are change , efficiency , performance of key essential steps , and the elimination of waste through small and continuous process improvements .
	manualset3
249956	8	425545	7	NULL	NULL	0	NULL	small improvements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounded productivity is the unique benefit of kaizen , and its principles are change , efficiency , performance of key essential steps , and the elimination of waste through small and continuous process improvements .
	manualset3
249958	9	425545	7	NULL	NULL	0	NULL	continuous process improvements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounded productivity is the unique benefit of kaizen , and its principles are change , efficiency , performance of key essential steps , and the elimination of waste through small and continuous process improvements .
	manualset3
249964	10	425545	7	NULL	NULL	0	NULL	performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounded productivity is the unique benefit of kaizen , and its principles are change , efficiency , performance of key essential steps , and the elimination of waste through small and continuous process improvements .
	manualset3
252908	11	425545	7	NULL	NULL	0	NULL	change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounded productivity is the unique benefit of kaizen , and its principles are change , efficiency , performance of key essential steps , and the elimination of waste through small and continuous process improvements .
	manualset3
252909	12	425545	7	NULL	NULL	0	NULL	 efficiency 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounded productivity is the unique benefit of kaizen , and its principles are change , efficiency , performance of key essential steps , and the elimination of waste through small and continuous process improvements .
	manualset3
250018	1	425546	7	NULL	NULL	0	NULL	Compounds ( ( 68 ) Ga ) 3 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounds ( ( 68 ) Ga ) 3 and ( ( 68 ) Ga ) 6 are high-affinity urea-based inhibitors of the prostate-specific membrane antigen ( PSMA ) that were synthesized in decay-uncorrected yields ranging from 60 % to 70 % and radiochemical purities of more than 99 % .
	manualset3
250019	2	425546	7	NULL	NULL	0	NULL	( ( 68 ) Ga ) 6	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounds ( ( 68 ) Ga ) 3 and ( ( 68 ) Ga ) 6 are high-affinity urea-based inhibitors of the prostate-specific membrane antigen ( PSMA ) that were synthesized in decay-uncorrected yields ranging from 60 % to 70 % and radiochemical purities of more than 99 % .
	manualset3
250020	3	425546	7	NULL	NULL	0	NULL	 high-affinity urea-based inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounds ( ( 68 ) Ga ) 3 and ( ( 68 ) Ga ) 6 are high-affinity urea-based inhibitors of the prostate-specific membrane antigen ( PSMA ) that were synthesized in decay-uncorrected yields ranging from 60 % to 70 % and radiochemical purities of more than 99 % .
	manualset3
250021	4	425546	7	NULL	NULL	0	NULL	prostate-specific membrane antigen ( PSMA )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounds ( ( 68 ) Ga ) 3 and ( ( 68 ) Ga ) 6 are high-affinity urea-based inhibitors of the prostate-specific membrane antigen ( PSMA ) that were synthesized in decay-uncorrected yields ranging from 60 % to 70 % and radiochemical purities of more than 99 % .
	manualset3
250022	5	425546	7	NULL	NULL	0	NULL	decay-uncorrected yields 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounds ( ( 68 ) Ga ) 3 and ( ( 68 ) Ga ) 6 are high-affinity urea-based inhibitors of the prostate-specific membrane antigen ( PSMA ) that were synthesized in decay-uncorrected yields ranging from 60 % to 70 % and radiochemical purities of more than 99 % .
	manualset3
250023	6	425546	7	NULL	NULL	0	NULL	60 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounds ( ( 68 ) Ga ) 3 and ( ( 68 ) Ga ) 6 are high-affinity urea-based inhibitors of the prostate-specific membrane antigen ( PSMA ) that were synthesized in decay-uncorrected yields ranging from 60 % to 70 % and radiochemical purities of more than 99 % .
	manualset3
250024	7	425546	7	NULL	NULL	0	NULL	 70 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounds ( ( 68 ) Ga ) 3 and ( ( 68 ) Ga ) 6 are high-affinity urea-based inhibitors of the prostate-specific membrane antigen ( PSMA ) that were synthesized in decay-uncorrected yields ranging from 60 % to 70 % and radiochemical purities of more than 99 % .
	manualset3
250026	8	425546	7	NULL	NULL	NULL	NULL	radiochemical purities	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Compounds ( ( 68 ) Ga ) 3 and ( ( 68 ) Ga ) 6 are high-affinity urea-based inhibitors of the prostate-specific membrane antigen ( PSMA ) that were synthesized in decay-uncorrected yields ranging from 60 % to 70 % and radiochemical purities of more than 99 % .
	manualset3
250027	9	425546	7	NULL	NULL	0	NULL	99 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounds ( ( 68 ) Ga ) 3 and ( ( 68 ) Ga ) 6 are high-affinity urea-based inhibitors of the prostate-specific membrane antigen ( PSMA ) that were synthesized in decay-uncorrected yields ranging from 60 % to 70 % and radiochemical purities of more than 99 % .
	manualset3
250030	1	425547	7	NULL	NULL	0	NULL	Compounds 10c	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounds 10c and 14 demonstrated broad-spectrum inhibition of the herpesvirus polymerases HCMV , HSV-1 , and VZV .
	manualset3
250031	2	425547	7	NULL	NULL	0	NULL	Compounds 14	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounds 10c and 14 demonstrated broad-spectrum inhibition of the herpesvirus polymerases HCMV , HSV-1 , and VZV .
	manualset3
250032	3	425547	7	NULL	NULL	0	NULL	 broad-spectrum inhibition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounds 10c and 14 demonstrated broad-spectrum inhibition of the herpesvirus polymerases HCMV , HSV-1 , and VZV .
	manualset3
250034	4	425547	7	NULL	NULL	0	NULL	herpesvirus polymerases HCMV	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounds 10c and 14 demonstrated broad-spectrum inhibition of the herpesvirus polymerases HCMV , HSV-1 , and VZV .
	manualset3
250036	5	425547	7	NULL	NULL	0	NULL	HSV-1	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounds 10c and 14 demonstrated broad-spectrum inhibition of the herpesvirus polymerases HCMV , HSV-1 , and VZV .
	manualset3
250037	6	425547	7	NULL	NULL	0	NULL	VZV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Compounds 10c and 14 demonstrated broad-spectrum inhibition of the herpesvirus polymerases HCMV , HSV-1 , and VZV .
	manualset3
250045	1	425548	7	NULL	NULL	0	NULL	KHK	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( KHK ) gave almost no suppression of P. aphanidermatum ( 7 % ) .
	manualset3
250047	2	425548	7	NULL	NULL	0	NULL	suppression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( KHK ) gave almost no suppression of P. aphanidermatum ( 7 % ) .
	manualset3
250049	3	425548	7	NULL	NULL	0	NULL	P. aphanidermatum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( KHK ) gave almost no suppression of P. aphanidermatum ( 7 % ) .
	manualset3
250050	4	425548	7	NULL	NULL	0	NULL	7 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( KHK ) gave almost no suppression of P. aphanidermatum ( 7 % ) .
	manualset3
250051	1	425549	7	NULL	NULL	0	NULL	Comprehensive information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Comprehensive information and appropriate use of pharmacologic agents for erectile dysfunction can add significantly to quality of life .
	manualset3
250052	2	425549	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Comprehensive information and appropriate use of pharmacologic agents for erectile dysfunction can add significantly to quality of life .
	manualset3
250053	3	425549	7	NULL	NULL	0	NULL	pharmacologic agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Comprehensive information and appropriate use of pharmacologic agents for erectile dysfunction can add significantly to quality of life .
	manualset3
250054	4	425549	7	NULL	NULL	0	NULL	erectile dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Comprehensive information and appropriate use of pharmacologic agents for erectile dysfunction can add significantly to quality of life .
	manualset3
250055	5	425549	7	NULL	NULL	0	NULL	quality	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comprehensive information and appropriate use of pharmacologic agents for erectile dysfunction can add significantly to quality of life .
	manualset3
250056	6	425549	7	NULL	NULL	0	NULL	 life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Comprehensive information and appropriate use of pharmacologic agents for erectile dysfunction can add significantly to quality of life .
	manualset3
250057	1	425550	7	NULL	NULL	0	NULL	Comprehensive surgical treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Comprehensive surgical and chemotherapy treatment for invasive bladder cancer .
	manualset3
250058	2	425550	7	NULL	NULL	0	NULL	chemotherapy treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Comprehensive surgical and chemotherapy treatment for invasive bladder cancer .
	manualset3
250059	3	425550	7	NULL	NULL	0	NULL	invasive bladder cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Comprehensive surgical and chemotherapy treatment for invasive bladder cancer .
	manualset3
250078	1	425551	7	NULL	NULL	0	NULL	Comprehensive transcriptome analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Comprehensive transcriptome analysis reveals novel genes involved in cardiac glycoside biosynthesis and mlncRNAs associated with secondary metabolism and stress response in Digitalis purpurea .
	manualset3
250082	2	425551	7	NULL	NULL	0	NULL	novel genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Comprehensive transcriptome analysis reveals novel genes involved in cardiac glycoside biosynthesis and mlncRNAs associated with secondary metabolism and stress response in Digitalis purpurea .
	manualset3
250086	3	425551	7	NULL	NULL	0	NULL	cardiac glycoside biosynthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Comprehensive transcriptome analysis reveals novel genes involved in cardiac glycoside biosynthesis and mlncRNAs associated with secondary metabolism and stress response in Digitalis purpurea .
	manualset3
250087	4	425551	7	NULL	NULL	0	NULL	mlncRNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Comprehensive transcriptome analysis reveals novel genes involved in cardiac glycoside biosynthesis and mlncRNAs associated with secondary metabolism and stress response in Digitalis purpurea .
	manualset3
250088	5	425551	7	NULL	NULL	0	NULL	secondary metabolism 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Comprehensive transcriptome analysis reveals novel genes involved in cardiac glycoside biosynthesis and mlncRNAs associated with secondary metabolism and stress response in Digitalis purpurea .
	manualset3
250089	6	425551	7	NULL	NULL	0	NULL	stress response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Comprehensive transcriptome analysis reveals novel genes involved in cardiac glycoside biosynthesis and mlncRNAs associated with secondary metabolism and stress response in Digitalis purpurea .
	manualset3
250090	7	425551	7	NULL	NULL	0	NULL	Digitalis purpurea	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Comprehensive transcriptome analysis reveals novel genes involved in cardiac glycoside biosynthesis and mlncRNAs associated with secondary metabolism and stress response in Digitalis purpurea .
	manualset3
250091	1	425552	7	NULL	NULL	0	NULL	Compression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Compression of medical images has always been viewed with skepticism , since the loss of information involved is thought to affect diagnostic information .
	manualset3
250092	2	425552	7	NULL	NULL	0	NULL	medical images	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Compression of medical images has always been viewed with skepticism , since the loss of information involved is thought to affect diagnostic information .
	manualset3
250093	3	425552	7	NULL	NULL	0	NULL	skepticism	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compression of medical images has always been viewed with skepticism , since the loss of information involved is thought to affect diagnostic information .
	manualset3
250094	4	425552	7	NULL	NULL	0	NULL	loss	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Compression of medical images has always been viewed with skepticism , since the loss of information involved is thought to affect diagnostic information .
	manualset3
250095	5	425552	7	NULL	NULL	0	NULL	information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Compression of medical images has always been viewed with skepticism , since the loss of information involved is thought to affect diagnostic information .
	manualset3
250096	6	425552	7	NULL	NULL	0	NULL	diagnostic information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Compression of medical images has always been viewed with skepticism , since the loss of information involved is thought to affect diagnostic information .
	manualset3
250097	1	425553	7	NULL	NULL	0	NULL	Computational dosimetry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Computational dosimetry of a simulated combined standard X-Rays and BNCT treatment .
	manualset3
250098	2	425553	7	NULL	NULL	0	NULL	simulated combined standard X-Rays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Computational dosimetry of a simulated combined standard X-Rays and BNCT treatment .
	manualset3
250099	3	425553	7	NULL	NULL	0	NULL	BNCT treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Computational dosimetry of a simulated combined standard X-Rays and BNCT treatment .
	manualset3
250100	1	425554	7	NULL	NULL	0	NULL	Computational models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Computational models were used to estimate hemodynamics and oxygen distribution and to simulate vascular diameter adaptation in response to hemodynamic , metabolic and conducted stimuli .
	manualset3
250101	2	425554	7	NULL	NULL	0	NULL	hemodynamics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Computational models were used to estimate hemodynamics and oxygen distribution and to simulate vascular diameter adaptation in response to hemodynamic , metabolic and conducted stimuli .
	manualset3
250102	3	425554	7	NULL	NULL	0	NULL	oxygen distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Computational models were used to estimate hemodynamics and oxygen distribution and to simulate vascular diameter adaptation in response to hemodynamic , metabolic and conducted stimuli .
	manualset3
250103	4	425554	7	NULL	NULL	0	NULL	vascular diameter adaptation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Computational models were used to estimate hemodynamics and oxygen distribution and to simulate vascular diameter adaptation in response to hemodynamic , metabolic and conducted stimuli .
	manualset3
250104	5	425554	7	NULL	NULL	0	NULL	hemodynamic stimuli	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Computational models were used to estimate hemodynamics and oxygen distribution and to simulate vascular diameter adaptation in response to hemodynamic , metabolic and conducted stimuli .
	manualset3
250105	6	425554	7	NULL	NULL	0	NULL	metabolic stimuli	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Computational models were used to estimate hemodynamics and oxygen distribution and to simulate vascular diameter adaptation in response to hemodynamic , metabolic and conducted stimuli .
	manualset3
250106	7	425554	7	NULL	NULL	0	NULL	conducted stimuli 	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Computational models were used to estimate hemodynamics and oxygen distribution and to simulate vascular diameter adaptation in response to hemodynamic , metabolic and conducted stimuli .
	manualset3
250107	1	425555	7	NULL	NULL	0	NULL	Computed tomography ( CT )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Computed tomography ( CT ) is superior to conventional radiography in the assessment of the position of fracture fragments and was used to study 20 patients with supracondylar fractures after reduction .
	manualset3
250108	2	425555	7	NULL	NULL	0	NULL	conventional radiography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Computed tomography ( CT ) is superior to conventional radiography in the assessment of the position of fracture fragments and was used to study 20 patients with supracondylar fractures after reduction .
	manualset3
250110	3	425555	7	NULL	NULL	0	NULL	 assessment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Computed tomography ( CT ) is superior to conventional radiography in the assessment of the position of fracture fragments and was used to study 20 patients with supracondylar fractures after reduction .
	manualset3
250111	4	425555	7	NULL	NULL	0	NULL	 position	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Computed tomography ( CT ) is superior to conventional radiography in the assessment of the position of fracture fragments and was used to study 20 patients with supracondylar fractures after reduction .
	manualset3
250112	5	425555	7	NULL	NULL	0	NULL	fracture fragments 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Computed tomography ( CT ) is superior to conventional radiography in the assessment of the position of fracture fragments and was used to study 20 patients with supracondylar fractures after reduction .
	manualset3
250113	6	425555	7	NULL	NULL	0	NULL	20 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Computed tomography ( CT ) is superior to conventional radiography in the assessment of the position of fracture fragments and was used to study 20 patients with supracondylar fractures after reduction .
	manualset3
250114	7	425555	7	NULL	NULL	0	NULL	supracondylar fractures 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Computed tomography ( CT ) is superior to conventional radiography in the assessment of the position of fracture fragments and was used to study 20 patients with supracondylar fractures after reduction .
	manualset3
250115	8	425555	7	NULL	NULL	0	NULL	 reduction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Computed tomography ( CT ) is superior to conventional radiography in the assessment of the position of fracture fragments and was used to study 20 patients with supracondylar fractures after reduction .
	manualset3
250116	1	425556	7	NULL	NULL	0	NULL	Kidney lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Kidney lesion in the Laurence-Moon-Bardet-Biedl syndrome ) .
	manualset3
250117	2	425556	7	NULL	NULL	0	NULL	Laurence-Moon-Bardet-Biedl syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Kidney lesion in the Laurence-Moon-Bardet-Biedl syndrome ) .
	manualset3
250118	1	425557	7	NULL	NULL	0	NULL	Computed tomography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Computed tomography revealed ascending aortic dilatation ( maximum diameter 64 mm ) complicated with aortic dissection .
	manualset3
250119	2	425557	7	NULL	NULL	NULL	NULL	ascending aortic dilatation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Computed tomography revealed ascending aortic dilatation ( maximum diameter 64 mm ) complicated with aortic dissection .
	manualset3
250120	3	425557	7	NULL	NULL	0	NULL	maximum diameter 64 mm	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Computed tomography revealed ascending aortic dilatation ( maximum diameter 64 mm ) complicated with aortic dissection .
	manualset3
250121	4	425557	7	NULL	NULL	0	NULL	aortic dissection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Computed tomography revealed ascending aortic dilatation ( maximum diameter 64 mm ) complicated with aortic dissection .
	manualset3
250122	1	425558	7	NULL	NULL	0	NULL	Computer-aided diagnosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Computer-aided diagnosis was made in three steps : registrations or selection of a patient , collection of history data and diagnosis , prescription of antiepileptic drugs .
	manualset3
250123	2	425558	7	NULL	NULL	0	NULL	three steps	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Computer-aided diagnosis was made in three steps : registrations or selection of a patient , collection of history data and diagnosis , prescription of antiepileptic drugs .
	manualset3
250124	3	425558	7	NULL	NULL	0	NULL	registrations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Computer-aided diagnosis was made in three steps : registrations or selection of a patient , collection of history data and diagnosis , prescription of antiepileptic drugs .
	manualset3
250125	4	425558	7	NULL	NULL	0	NULL	 selection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Computer-aided diagnosis was made in three steps : registrations or selection of a patient , collection of history data and diagnosis , prescription of antiepileptic drugs .
	manualset3
250126	5	425558	7	NULL	NULL	0	NULL	 patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Computer-aided diagnosis was made in three steps : registrations or selection of a patient , collection of history data and diagnosis , prescription of antiepileptic drugs .
	manualset3
250127	6	425558	7	NULL	NULL	0	NULL	collection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Computer-aided diagnosis was made in three steps : registrations or selection of a patient , collection of history data and diagnosis , prescription of antiepileptic drugs .
	manualset3
250128	7	425558	7	NULL	NULL	0	NULL	history data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Computer-aided diagnosis was made in three steps : registrations or selection of a patient , collection of history data and diagnosis , prescription of antiepileptic drugs .
	manualset3
250129	8	425558	7	NULL	NULL	0	NULL	 diagnosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Computer-aided diagnosis was made in three steps : registrations or selection of a patient , collection of history data and diagnosis , prescription of antiepileptic drugs .
	manualset3
250130	9	425558	7	NULL	NULL	0	NULL	prescription	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Computer-aided diagnosis was made in three steps : registrations or selection of a patient , collection of history data and diagnosis , prescription of antiepileptic drugs .
	manualset3
250131	10	425558	7	NULL	NULL	0	NULL	antiepileptic drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Computer-aided diagnosis was made in three steps : registrations or selection of a patient , collection of history data and diagnosis , prescription of antiepileptic drugs .
	manualset3
250132	1	425559	7	NULL	NULL	0	NULL	Computer evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Computer evaluation of peak isometric tension and resting tension of isolated myocardial muscle strip .
	manualset3
250133	2	425559	7	NULL	NULL	0	NULL	peak isometric tension	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Computer evaluation of peak isometric tension and resting tension of isolated myocardial muscle strip .
	manualset3
250134	3	425559	7	NULL	NULL	0	NULL	resting tension	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Computer evaluation of peak isometric tension and resting tension of isolated myocardial muscle strip .
	manualset3
250135	4	425559	7	NULL	NULL	0	NULL	isolated myocardial muscle strip	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Computer evaluation of peak isometric tension and resting tension of isolated myocardial muscle strip .
	manualset3
250136	1	425560	7	NULL	NULL	0	NULL	Computer modeling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Computer modeling of the shapes of the fluorescence distributions show that at 600 rad 30 to 40 % of the sperm have abnormal DNA content .
	manualset3
250137	2	425560	7	NULL	NULL	0	NULL	 shapes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Computer modeling of the shapes of the fluorescence distributions show that at 600 rad 30 to 40 % of the sperm have abnormal DNA content .
	manualset3
250138	3	425560	7	NULL	NULL	0	NULL	 fluorescence distributions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Computer modeling of the shapes of the fluorescence distributions show that at 600 rad 30 to 40 % of the sperm have abnormal DNA content .
	manualset3
250139	4	425560	7	NULL	NULL	0	NULL	600 rad 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Computer modeling of the shapes of the fluorescence distributions show that at 600 rad 30 to 40 % of the sperm have abnormal DNA content .
	manualset3
250140	5	425560	7	NULL	NULL	0	NULL	30%	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Computer modeling of the shapes of the fluorescence distributions show that at 600 rad 30 to 40 % of the sperm have abnormal DNA content .
	manualset3
250141	6	425560	7	NULL	NULL	0	NULL	40 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Computer modeling of the shapes of the fluorescence distributions show that at 600 rad 30 to 40 % of the sperm have abnormal DNA content .
	manualset3
250142	7	425560	7	NULL	NULL	0	NULL	sperm	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Computer modeling of the shapes of the fluorescence distributions show that at 600 rad 30 to 40 % of the sperm have abnormal DNA content .
	manualset3
250143	8	425560	7	NULL	NULL	0	NULL	abnormal DNA content 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Computer modeling of the shapes of the fluorescence distributions show that at 600 rad 30 to 40 % of the sperm have abnormal DNA content .
	manualset3
250145	1	425561	7	NULL	NULL	0	NULL	Computer simulated screening	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Computer simulated screening of dentin bonding primer monomers through analysis of their chemical functions and their spatial 3D alignment .
	manualset3
250146	2	425561	7	NULL	NULL	0	NULL	dentin bonding primer monomers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Computer simulated screening of dentin bonding primer monomers through analysis of their chemical functions and their spatial 3D alignment .
	manualset3
250147	3	425561	7	NULL	NULL	0	NULL	analysis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Computer simulated screening of dentin bonding primer monomers through analysis of their chemical functions and their spatial 3D alignment .
	manualset3
250148	4	425561	7	NULL	NULL	0	NULL	chemical functions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Computer simulated screening of dentin bonding primer monomers through analysis of their chemical functions and their spatial 3D alignment .
	manualset3
250149	5	425561	7	NULL	NULL	0	NULL	spatial 3D alignment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Computer simulated screening of dentin bonding primer monomers through analysis of their chemical functions and their spatial 3D alignment .
	manualset3
250150	1	425562	7	NULL	NULL	NULL	NULL	Computer simulation	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Computer simulation of wild-type and mutant human cardiac Na + current .
	manualset3
250151	2	425562	7	NULL	NULL	NULL	NULL	wild-type human cardiac Na + current 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Computer simulation of wild-type and mutant human cardiac Na + current .
	manualset3
250152	3	425562	7	NULL	NULL	NULL	NULL	mutant human cardiac Na + current 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Computer simulation of wild-type and mutant human cardiac Na + current .
	manualset3
250153	1	425563	7	NULL	NULL	0	NULL	Computer use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Computer use , computer training , and employment .
	manualset3
250154	2	425563	7	NULL	NULL	0	NULL	computer training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Computer use , computer training , and employment .
	manualset3
250155	3	425563	7	NULL	NULL	0	NULL	employment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Computer use , computer training , and employment .
	manualset3
250156	1	425564	7	NULL	NULL	0	NULL	Kinetics	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Kinetics of mezlocillin in injured subjects ) .
	manualset3
250157	2	425564	7	NULL	NULL	0	NULL	mezlocillin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Kinetics of mezlocillin in injured subjects ) .
	manualset3
250158	3	425564	7	NULL	NULL	0	NULL	injured subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Kinetics of mezlocillin in injured subjects ) .
	manualset3
250159	1	425565	7	NULL	NULL	0	NULL	Computerized lung acoustic monitoring 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Computerized lung acoustic monitoring can help to differentiate between various chest radiographic densities in critically ill patients .
	manualset3
250160	2	425565	7	NULL	NULL	0	NULL	chest radiographic densities 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Computerized lung acoustic monitoring can help to differentiate between various chest radiographic densities in critically ill patients .
	manualset3
250161	3	425565	7	NULL	NULL	0	NULL	 ill patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Computerized lung acoustic monitoring can help to differentiate between various chest radiographic densities in critically ill patients .
	manualset3
250162	1	425566	7	NULL	NULL	0	NULL	Computerized tomography ( CT )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Computerized tomography ( CT ) correctly predicted the presence of a thymoma in one patient and falsely predicted a thymoma in a patient with a thymic cyst ; it accurately predicted the absence of a thymoma in the remaining 11 patients .
	manualset3
250163	2	425566	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Computerized tomography ( CT ) correctly predicted the presence of a thymoma in one patient and falsely predicted a thymoma in a patient with a thymic cyst ; it accurately predicted the absence of a thymoma in the remaining 11 patients .
	manualset3
250164	3	425566	7	NULL	NULL	0	NULL	thymoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Computerized tomography ( CT ) correctly predicted the presence of a thymoma in one patient and falsely predicted a thymoma in a patient with a thymic cyst ; it accurately predicted the absence of a thymoma in the remaining 11 patients .
	manualset3
250165	4	425566	7	NULL	NULL	0	NULL	one patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Computerized tomography ( CT ) correctly predicted the presence of a thymoma in one patient and falsely predicted a thymoma in a patient with a thymic cyst ; it accurately predicted the absence of a thymoma in the remaining 11 patients .
	manualset3
250166	5	425566	7	NULL	NULL	0	NULL	thymoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Computerized tomography ( CT ) correctly predicted the presence of a thymoma in one patient and falsely predicted a thymoma in a patient with a thymic cyst ; it accurately predicted the absence of a thymoma in the remaining 11 patients .
	manualset3
250167	6	425566	7	NULL	NULL	0	NULL	 patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Computerized tomography ( CT ) correctly predicted the presence of a thymoma in one patient and falsely predicted a thymoma in a patient with a thymic cyst ; it accurately predicted the absence of a thymoma in the remaining 11 patients .
	manualset3
250168	7	425566	7	NULL	NULL	0	NULL	thymic cyst	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Computerized tomography ( CT ) correctly predicted the presence of a thymoma in one patient and falsely predicted a thymoma in a patient with a thymic cyst ; it accurately predicted the absence of a thymoma in the remaining 11 patients .
	manualset3
250169	8	425566	7	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Computerized tomography ( CT ) correctly predicted the presence of a thymoma in one patient and falsely predicted a thymoma in a patient with a thymic cyst ; it accurately predicted the absence of a thymoma in the remaining 11 patients .
	manualset3
250170	9	425566	7	NULL	NULL	0	NULL	thymoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Computerized tomography ( CT ) correctly predicted the presence of a thymoma in one patient and falsely predicted a thymoma in a patient with a thymic cyst ; it accurately predicted the absence of a thymoma in the remaining 11 patients .
	manualset3
250171	10	425566	7	NULL	NULL	0	NULL	11 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Computerized tomography ( CT ) correctly predicted the presence of a thymoma in one patient and falsely predicted a thymoma in a patient with a thymic cyst ; it accurately predicted the absence of a thymoma in the remaining 11 patients .
	manualset3
250172	1	425567	7	NULL	NULL	0	NULL	Con-R	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Con-R prevented sound-induced tonic extension seizures in the Frings audiogenic seizure-susceptible mice at i.c.v. doses below toxic levels .
	manualset3
250173	2	425567	7	NULL	NULL	0	NULL	sound-induced tonic extension seizures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Con-R prevented sound-induced tonic extension seizures in the Frings audiogenic seizure-susceptible mice at i.c.v. doses below toxic levels .
	manualset3
250174	3	425567	7	NULL	NULL	0	NULL	Frings audiogenic seizure-susceptible mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Con-R prevented sound-induced tonic extension seizures in the Frings audiogenic seizure-susceptible mice at i.c.v. doses below toxic levels .
	manualset3
250175	4	425567	7	NULL	NULL	0	NULL	 i.c.v. doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Con-R prevented sound-induced tonic extension seizures in the Frings audiogenic seizure-susceptible mice at i.c.v. doses below toxic levels .
	manualset3
250176	5	425567	7	NULL	NULL	NULL	NULL	toxic levels	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Con-R prevented sound-induced tonic extension seizures in the Frings audiogenic seizure-susceptible mice at i.c.v. doses below toxic levels .
	manualset3
250177	1	425568	7	NULL	NULL	0	NULL	Concatamerization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Concatamerization of simple repeat oligomers further enables the use of relatively short oligonucleotide sequences in direct-label chemiluminescent hybridization experiments , thereby reducing the overall need for radioisotopes in certain commonly performed laboratory procedures such as DNA fingerprinting and selection of clones containing microsatellite sequences .
	manualset3
250178	2	425568	7	NULL	NULL	0	NULL	simple repeat oligomers	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Concatamerization of simple repeat oligomers further enables the use of relatively short oligonucleotide sequences in direct-label chemiluminescent hybridization experiments , thereby reducing the overall need for radioisotopes in certain commonly performed laboratory procedures such as DNA fingerprinting and selection of clones containing microsatellite sequences .
	manualset3
250179	3	425568	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Concatamerization of simple repeat oligomers further enables the use of relatively short oligonucleotide sequences in direct-label chemiluminescent hybridization experiments , thereby reducing the overall need for radioisotopes in certain commonly performed laboratory procedures such as DNA fingerprinting and selection of clones containing microsatellite sequences .
	manualset3
250180	4	425568	7	NULL	NULL	0	NULL	short oligonucleotide sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Concatamerization of simple repeat oligomers further enables the use of relatively short oligonucleotide sequences in direct-label chemiluminescent hybridization experiments , thereby reducing the overall need for radioisotopes in certain commonly performed laboratory procedures such as DNA fingerprinting and selection of clones containing microsatellite sequences .
	manualset3
250181	5	425568	7	NULL	NULL	0	NULL	direct-label chemiluminescent hybridization experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concatamerization of simple repeat oligomers further enables the use of relatively short oligonucleotide sequences in direct-label chemiluminescent hybridization experiments , thereby reducing the overall need for radioisotopes in certain commonly performed laboratory procedures such as DNA fingerprinting and selection of clones containing microsatellite sequences .
	manualset3
250183	7	425568	7	NULL	NULL	0	NULL	radioisotopes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Concatamerization of simple repeat oligomers further enables the use of relatively short oligonucleotide sequences in direct-label chemiluminescent hybridization experiments , thereby reducing the overall need for radioisotopes in certain commonly performed laboratory procedures such as DNA fingerprinting and selection of clones containing microsatellite sequences .
	manualset3
250184	8	425568	7	NULL	NULL	NULL	NULL	laboratory procedures	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Concatamerization of simple repeat oligomers further enables the use of relatively short oligonucleotide sequences in direct-label chemiluminescent hybridization experiments , thereby reducing the overall need for radioisotopes in certain commonly performed laboratory procedures such as DNA fingerprinting and selection of clones containing microsatellite sequences .
	manualset3
250185	9	425568	7	NULL	NULL	0	NULL	DNA fingerprinting	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concatamerization of simple repeat oligomers further enables the use of relatively short oligonucleotide sequences in direct-label chemiluminescent hybridization experiments , thereby reducing the overall need for radioisotopes in certain commonly performed laboratory procedures such as DNA fingerprinting and selection of clones containing microsatellite sequences .
	manualset3
250186	10	425568	7	NULL	NULL	0	NULL	selection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Concatamerization of simple repeat oligomers further enables the use of relatively short oligonucleotide sequences in direct-label chemiluminescent hybridization experiments , thereby reducing the overall need for radioisotopes in certain commonly performed laboratory procedures such as DNA fingerprinting and selection of clones containing microsatellite sequences .
	manualset3
250187	11	425568	7	NULL	NULL	0	NULL	clones	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Concatamerization of simple repeat oligomers further enables the use of relatively short oligonucleotide sequences in direct-label chemiluminescent hybridization experiments , thereby reducing the overall need for radioisotopes in certain commonly performed laboratory procedures such as DNA fingerprinting and selection of clones containing microsatellite sequences .
	manualset3
250188	12	425568	7	NULL	NULL	0	NULL	microsatellite sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Concatamerization of simple repeat oligomers further enables the use of relatively short oligonucleotide sequences in direct-label chemiluminescent hybridization experiments , thereby reducing the overall need for radioisotopes in certain commonly performed laboratory procedures such as DNA fingerprinting and selection of clones containing microsatellite sequences .
	manualset3
252910	13	425568	7	NULL	NULL	0	NULL	need	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Concatamerization of simple repeat oligomers further enables the use of relatively short oligonucleotide sequences in direct-label chemiluminescent hybridization experiments , thereby reducing the overall need for radioisotopes in certain commonly performed laboratory procedures such as DNA fingerprinting and selection of clones containing microsatellite sequences .
	manualset3
250189	1	425569	7	NULL	NULL	0	NULL	Concealing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Concealing was well planned to avoid such fear , and to preserve dignity .
	manualset3
250190	2	425569	7	NULL	NULL	0	NULL	 fear	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Concealing was well planned to avoid such fear , and to preserve dignity .
	manualset3
250191	3	425569	7	NULL	NULL	0	NULL	 dignity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Concealing was well planned to avoid such fear , and to preserve dignity .
	manualset3
250192	1	425570	7	NULL	NULL	0	NULL	Concentration 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentration of marine and freshwater samples was done by adsorption/elution followed by molecular detection by ( RT ) - PCR .
	manualset3
250193	2	425570	7	NULL	NULL	0	NULL	marine samples	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentration of marine and freshwater samples was done by adsorption/elution followed by molecular detection by ( RT ) - PCR .
	manualset3
250194	3	425570	7	NULL	NULL	0	NULL	freshwater samples	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentration of marine and freshwater samples was done by adsorption/elution followed by molecular detection by ( RT ) - PCR .
	manualset3
250195	4	425570	7	NULL	NULL	0	NULL	adsorption/elution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentration of marine and freshwater samples was done by adsorption/elution followed by molecular detection by ( RT ) - PCR .
	manualset3
250196	5	425570	7	NULL	NULL	0	NULL	molecular detection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentration of marine and freshwater samples was done by adsorption/elution followed by molecular detection by ( RT ) - PCR .
	manualset3
250197	6	425570	7	NULL	NULL	0	NULL	( RT ) - PCR	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentration of marine and freshwater samples was done by adsorption/elution followed by molecular detection by ( RT ) - PCR .
	manualset3
250198	1	425571	7	NULL	NULL	NULL	NULL	Concentrations	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Concentrations and distribution of chlorinated hydrocarbon insecticides , polychlorinated biphenyls ( PCB 's ) and some metals were determined in two South African lakes , Hartbeespoort Dam and Volvlei Dam .
	manualset3
250199	2	425571	7	NULL	NULL	0	NULL	distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations and distribution of chlorinated hydrocarbon insecticides , polychlorinated biphenyls ( PCB 's ) and some metals were determined in two South African lakes , Hartbeespoort Dam and Volvlei Dam .
	manualset3
250200	3	425571	7	NULL	NULL	0	NULL	chlorinated hydrocarbon insecticides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations and distribution of chlorinated hydrocarbon insecticides , polychlorinated biphenyls ( PCB 's ) and some metals were determined in two South African lakes , Hartbeespoort Dam and Volvlei Dam .
	manualset3
250201	4	425571	7	NULL	NULL	0	NULL	polychlorinated biphenyls ( PCB 's )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations and distribution of chlorinated hydrocarbon insecticides , polychlorinated biphenyls ( PCB 's ) and some metals were determined in two South African lakes , Hartbeespoort Dam and Volvlei Dam .
	manualset3
250202	5	425571	7	NULL	NULL	0	NULL	metals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations and distribution of chlorinated hydrocarbon insecticides , polychlorinated biphenyls ( PCB 's ) and some metals were determined in two South African lakes , Hartbeespoort Dam and Volvlei Dam .
	manualset3
250203	6	425571	7	NULL	NULL	0	NULL	 two South African lakes	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations and distribution of chlorinated hydrocarbon insecticides , polychlorinated biphenyls ( PCB 's ) and some metals were determined in two South African lakes , Hartbeespoort Dam and Volvlei Dam .
	manualset3
250204	7	425571	7	NULL	NULL	0	NULL	Hartbeespoort Dam	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations and distribution of chlorinated hydrocarbon insecticides , polychlorinated biphenyls ( PCB 's ) and some metals were determined in two South African lakes , Hartbeespoort Dam and Volvlei Dam .
	manualset3
250205	8	425571	7	NULL	NULL	0	NULL	Volvlei Dam	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations and distribution of chlorinated hydrocarbon insecticides , polychlorinated biphenyls ( PCB 's ) and some metals were determined in two South African lakes , Hartbeespoort Dam and Volvlei Dam .
	manualset3
250206	1	425572	7	NULL	NULL	0	NULL	Concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations for suppression of 50 and 90 % population growth and eradication ( rC0 ) of mites were fit to linear regression models .
	manualset3
250207	2	425572	7	NULL	NULL	0	NULL	suppression	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations for suppression of 50 and 90 % population growth and eradication ( rC0 ) of mites were fit to linear regression models .
	manualset3
250208	3	425572	7	NULL	NULL	0	NULL	50 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations for suppression of 50 and 90 % population growth and eradication ( rC0 ) of mites were fit to linear regression models .
	manualset3
250209	4	425572	7	NULL	NULL	0	NULL	90 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations for suppression of 50 and 90 % population growth and eradication ( rC0 ) of mites were fit to linear regression models .
	manualset3
250210	5	425572	7	NULL	NULL	0	NULL	population growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations for suppression of 50 and 90 % population growth and eradication ( rC0 ) of mites were fit to linear regression models .
	manualset3
250211	6	425572	7	NULL	NULL	0	NULL	eradication ( rC0 )	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations for suppression of 50 and 90 % population growth and eradication ( rC0 ) of mites were fit to linear regression models .
	manualset3
250212	7	425572	7	NULL	NULL	0	NULL	mites	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations for suppression of 50 and 90 % population growth and eradication ( rC0 ) of mites were fit to linear regression models .
	manualset3
250213	8	425572	7	NULL	NULL	0	NULL	 linear regression models	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations for suppression of 50 and 90 % population growth and eradication ( rC0 ) of mites were fit to linear regression models .
	manualset3
250219	1	425573	7	NULL	NULL	0	NULL	Concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of EE2 were tested at 1 , 3 , or 10 ng/L for 30 d from fertilization or during only the last 4 d with dimethylsulfoxide ( DMSO ) as presolvent ( 0.01 % ) .
	manualset3
250227	3	425573	7	NULL	NULL	0	NULL	EE2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of EE2 were tested at 1 , 3 , or 10 ng/L for 30 d from fertilization or during only the last 4 d with dimethylsulfoxide ( DMSO ) as presolvent ( 0.01 % ) .
	manualset3
250228	4	425573	7	NULL	NULL	0	NULL	 1 ng/L	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of EE2 were tested at 1 , 3 , or 10 ng/L for 30 d from fertilization or during only the last 4 d with dimethylsulfoxide ( DMSO ) as presolvent ( 0.01 % ) .
	manualset3
250229	5	425573	7	NULL	NULL	0	NULL	 3 ng/L 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of EE2 were tested at 1 , 3 , or 10 ng/L for 30 d from fertilization or during only the last 4 d with dimethylsulfoxide ( DMSO ) as presolvent ( 0.01 % ) .
	manualset3
250231	6	425573	7	NULL	NULL	0	NULL	10 ng/L	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of EE2 were tested at 1 , 3 , or 10 ng/L for 30 d from fertilization or during only the last 4 d with dimethylsulfoxide ( DMSO ) as presolvent ( 0.01 % ) .
	manualset3
250232	7	425573	7	NULL	NULL	0	NULL	30 d	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of EE2 were tested at 1 , 3 , or 10 ng/L for 30 d from fertilization or during only the last 4 d with dimethylsulfoxide ( DMSO ) as presolvent ( 0.01 % ) .
	manualset3
250233	8	425573	7	NULL	NULL	0	NULL	fertilization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of EE2 were tested at 1 , 3 , or 10 ng/L for 30 d from fertilization or during only the last 4 d with dimethylsulfoxide ( DMSO ) as presolvent ( 0.01 % ) .
	manualset3
250234	9	425573	7	NULL	NULL	0	NULL	 4 d	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of EE2 were tested at 1 , 3 , or 10 ng/L for 30 d from fertilization or during only the last 4 d with dimethylsulfoxide ( DMSO ) as presolvent ( 0.01 % ) .
	manualset3
250235	10	425573	7	NULL	NULL	0	NULL	dimethylsulfoxide ( DMSO )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of EE2 were tested at 1 , 3 , or 10 ng/L for 30 d from fertilization or during only the last 4 d with dimethylsulfoxide ( DMSO ) as presolvent ( 0.01 % ) .
	manualset3
250236	11	425573	7	NULL	NULL	0	NULL	presolvent ( 0.01 % )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of EE2 were tested at 1 , 3 , or 10 ng/L for 30 d from fertilization or during only the last 4 d with dimethylsulfoxide ( DMSO ) as presolvent ( 0.01 % ) .
	manualset3
250237	1	425574	7	NULL	NULL	0	NULL	Kymographic observation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Kymographic observation of pulse-synchronous movement of the spleen ) .
	manualset3
250238	2	425574	7	NULL	NULL	0	NULL	 pulse-synchronous movement	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Kymographic observation of pulse-synchronous movement of the spleen ) .
	manualset3
250239	3	425574	7	NULL	NULL	0	NULL	spleen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Kymographic observation of pulse-synchronous movement of the spleen ) .
	manualset3
250267	1	425575	7	NULL	NULL	0	NULL	Concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of LH from 42 to 84 d of age were more highly correlated with testicular traits than were the concentrations from 98 to 140 d. ( ABSTRACT TRUNCATED AT 250 WORDS )
	manualset3
250268	2	425575	7	NULL	NULL	0	NULL	LH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of LH from 42 to 84 d of age were more highly correlated with testicular traits than were the concentrations from 98 to 140 d. ( ABSTRACT TRUNCATED AT 250 WORDS )
	manualset3
250269	3	425575	7	NULL	NULL	NULL	NULL	42 d	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Concentrations of LH from 42 to 84 d of age were more highly correlated with testicular traits than were the concentrations from 98 to 140 d. ( ABSTRACT TRUNCATED AT 250 WORDS )
	manualset3
250270	4	425575	7	NULL	NULL	0	NULL	84 d	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of LH from 42 to 84 d of age were more highly correlated with testicular traits than were the concentrations from 98 to 140 d. ( ABSTRACT TRUNCATED AT 250 WORDS )
	manualset3
250271	5	425575	7	NULL	NULL	0	NULL	age	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of LH from 42 to 84 d of age were more highly correlated with testicular traits than were the concentrations from 98 to 140 d. ( ABSTRACT TRUNCATED AT 250 WORDS )
	manualset3
250272	6	425575	7	NULL	NULL	0	NULL	testicular traits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of LH from 42 to 84 d of age were more highly correlated with testicular traits than were the concentrations from 98 to 140 d. ( ABSTRACT TRUNCATED AT 250 WORDS )
	manualset3
250273	7	425575	7	NULL	NULL	0	NULL	 concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of LH from 42 to 84 d of age were more highly correlated with testicular traits than were the concentrations from 98 to 140 d. ( ABSTRACT TRUNCATED AT 250 WORDS )
	manualset3
250274	8	425575	7	NULL	NULL	0	NULL	98 d	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of LH from 42 to 84 d of age were more highly correlated with testicular traits than were the concentrations from 98 to 140 d. ( ABSTRACT TRUNCATED AT 250 WORDS )
	manualset3
250275	9	425575	7	NULL	NULL	0	NULL	 140 d	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of LH from 42 to 84 d of age were more highly correlated with testicular traits than were the concentrations from 98 to 140 d. ( ABSTRACT TRUNCATED AT 250 WORDS )
	manualset3
250276	10	425575	7	NULL	NULL	0	NULL	ABSTRACT	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of LH from 42 to 84 d of age were more highly correlated with testicular traits than were the concentrations from 98 to 140 d. ( ABSTRACT TRUNCATED AT 250 WORDS )
	manualset3
250277	11	425575	7	NULL	NULL	0	NULL	250 WORDS	Language												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of LH from 42 to 84 d of age were more highly correlated with testicular traits than were the concentrations from 98 to 140 d. ( ABSTRACT TRUNCATED AT 250 WORDS )
	manualset3
250278	1	425576	7	NULL	NULL	0	NULL	Concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of five metals ( cadmium , chromium , copper , nickel and lead ) were determined in tree leaves collected from 13 areas of the Attica basin and Athens city , Greece .
	manualset3
250279	2	425576	7	NULL	NULL	0	NULL	five metals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of five metals ( cadmium , chromium , copper , nickel and lead ) were determined in tree leaves collected from 13 areas of the Attica basin and Athens city , Greece .
	manualset3
250280	3	425576	7	NULL	NULL	0	NULL	 cadmium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of five metals ( cadmium , chromium , copper , nickel and lead ) were determined in tree leaves collected from 13 areas of the Attica basin and Athens city , Greece .
	manualset3
250281	4	425576	7	NULL	NULL	0	NULL	chromium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of five metals ( cadmium , chromium , copper , nickel and lead ) were determined in tree leaves collected from 13 areas of the Attica basin and Athens city , Greece .
	manualset3
250282	5	425576	7	NULL	NULL	0	NULL	copper	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of five metals ( cadmium , chromium , copper , nickel and lead ) were determined in tree leaves collected from 13 areas of the Attica basin and Athens city , Greece .
	manualset3
250283	6	425576	7	NULL	NULL	0	NULL	nickel	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of five metals ( cadmium , chromium , copper , nickel and lead ) were determined in tree leaves collected from 13 areas of the Attica basin and Athens city , Greece .
	manualset3
250284	7	425576	7	NULL	NULL	0	NULL	lead	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of five metals ( cadmium , chromium , copper , nickel and lead ) were determined in tree leaves collected from 13 areas of the Attica basin and Athens city , Greece .
	manualset3
250286	8	425576	7	NULL	NULL	NULL	NULL	tree leaves	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Concentrations of five metals ( cadmium , chromium , copper , nickel and lead ) were determined in tree leaves collected from 13 areas of the Attica basin and Athens city , Greece .
	manualset3
250292	9	425576	7	NULL	NULL	0	NULL	13 areas	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of five metals ( cadmium , chromium , copper , nickel and lead ) were determined in tree leaves collected from 13 areas of the Attica basin and Athens city , Greece .
	manualset3
250294	10	425576	7	NULL	NULL	0	NULL	Attica basin	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of five metals ( cadmium , chromium , copper , nickel and lead ) were determined in tree leaves collected from 13 areas of the Attica basin and Athens city , Greece .
	manualset3
250295	11	425576	7	NULL	NULL	0	NULL	Athens city	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of five metals ( cadmium , chromium , copper , nickel and lead ) were determined in tree leaves collected from 13 areas of the Attica basin and Athens city , Greece .
	manualset3
250296	12	425576	7	NULL	NULL	0	NULL	Greece	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of five metals ( cadmium , chromium , copper , nickel and lead ) were determined in tree leaves collected from 13 areas of the Attica basin and Athens city , Greece .
	manualset3
250430	1	425577	7	NULL	NULL	0	NULL	Concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of glutamine ( 902 micromol/L ) , glycine ( 24 micromol/L ) and alanine ( 78 micromol/L ) were elevated in CSF .
	manualset3
250431	2	425577	7	NULL	NULL	NULL	NULL	 glutamine	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Concentrations of glutamine ( 902 micromol/L ) , glycine ( 24 micromol/L ) and alanine ( 78 micromol/L ) were elevated in CSF .
	manualset3
250432	3	425577	7	NULL	NULL	0	NULL	902 micromol/L	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of glutamine ( 902 micromol/L ) , glycine ( 24 micromol/L ) and alanine ( 78 micromol/L ) were elevated in CSF .
	manualset3
250433	4	425577	7	NULL	NULL	0	NULL	 glycine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of glutamine ( 902 micromol/L ) , glycine ( 24 micromol/L ) and alanine ( 78 micromol/L ) were elevated in CSF .
	manualset3
250434	5	425577	7	NULL	NULL	0	NULL	24 micromol/L	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of glutamine ( 902 micromol/L ) , glycine ( 24 micromol/L ) and alanine ( 78 micromol/L ) were elevated in CSF .
	manualset3
250435	6	425577	7	NULL	NULL	0	NULL	alanine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of glutamine ( 902 micromol/L ) , glycine ( 24 micromol/L ) and alanine ( 78 micromol/L ) were elevated in CSF .
	manualset3
250436	7	425577	7	NULL	NULL	0	NULL	78 micromol/L	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of glutamine ( 902 micromol/L ) , glycine ( 24 micromol/L ) and alanine ( 78 micromol/L ) were elevated in CSF .
	manualset3
250437	8	425577	7	NULL	NULL	0	NULL	CSF	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of glutamine ( 902 micromol/L ) , glycine ( 24 micromol/L ) and alanine ( 78 micromol/L ) were elevated in CSF .
	manualset3
250438	1	425578	7	NULL	NULL	0	NULL	Concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of the inducers producing death of 48-66 % of Raji cells were determined to be : for dsRNA , 200 micrograms/ml ; polyguacyl , 400 micrograms/ml ; tiloron , 100 micrograms/ml ; Tash-4 , 200 micrograms/ml , which corresponded to the antiproliferative effect of 200 units/ml of alpha-interferon and 40 units/ml of gamma-interferon .
	manualset3
250439	2	425578	7	NULL	NULL	NULL	NULL	 inducers	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Concentrations of the inducers producing death of 48-66 % of Raji cells were determined to be : for dsRNA , 200 micrograms/ml ; polyguacyl , 400 micrograms/ml ; tiloron , 100 micrograms/ml ; Tash-4 , 200 micrograms/ml , which corresponded to the antiproliferative effect of 200 units/ml of alpha-interferon and 40 units/ml of gamma-interferon .
	manualset3
250440	3	425578	7	NULL	NULL	0	NULL	death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of the inducers producing death of 48-66 % of Raji cells were determined to be : for dsRNA , 200 micrograms/ml ; polyguacyl , 400 micrograms/ml ; tiloron , 100 micrograms/ml ; Tash-4 , 200 micrograms/ml , which corresponded to the antiproliferative effect of 200 units/ml of alpha-interferon and 40 units/ml of gamma-interferon .
	manualset3
250441	4	425578	7	NULL	NULL	0	NULL	48%	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of the inducers producing death of 48-66 % of Raji cells were determined to be : for dsRNA , 200 micrograms/ml ; polyguacyl , 400 micrograms/ml ; tiloron , 100 micrograms/ml ; Tash-4 , 200 micrograms/ml , which corresponded to the antiproliferative effect of 200 units/ml of alpha-interferon and 40 units/ml of gamma-interferon .
	manualset3
250442	5	425578	7	NULL	NULL	0	NULL	66 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of the inducers producing death of 48-66 % of Raji cells were determined to be : for dsRNA , 200 micrograms/ml ; polyguacyl , 400 micrograms/ml ; tiloron , 100 micrograms/ml ; Tash-4 , 200 micrograms/ml , which corresponded to the antiproliferative effect of 200 units/ml of alpha-interferon and 40 units/ml of gamma-interferon .
	manualset3
250443	6	425578	7	NULL	NULL	0	NULL	Raji cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of the inducers producing death of 48-66 % of Raji cells were determined to be : for dsRNA , 200 micrograms/ml ; polyguacyl , 400 micrograms/ml ; tiloron , 100 micrograms/ml ; Tash-4 , 200 micrograms/ml , which corresponded to the antiproliferative effect of 200 units/ml of alpha-interferon and 40 units/ml of gamma-interferon .
	manualset3
250444	7	425578	7	NULL	NULL	0	NULL	dsRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of the inducers producing death of 48-66 % of Raji cells were determined to be : for dsRNA , 200 micrograms/ml ; polyguacyl , 400 micrograms/ml ; tiloron , 100 micrograms/ml ; Tash-4 , 200 micrograms/ml , which corresponded to the antiproliferative effect of 200 units/ml of alpha-interferon and 40 units/ml of gamma-interferon .
	manualset3
250445	8	425578	7	NULL	NULL	0	NULL	200 micrograms/ml	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of the inducers producing death of 48-66 % of Raji cells were determined to be : for dsRNA , 200 micrograms/ml ; polyguacyl , 400 micrograms/ml ; tiloron , 100 micrograms/ml ; Tash-4 , 200 micrograms/ml , which corresponded to the antiproliferative effect of 200 units/ml of alpha-interferon and 40 units/ml of gamma-interferon .
	manualset3
250446	9	425578	7	NULL	NULL	0	NULL	 polyguacyl	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of the inducers producing death of 48-66 % of Raji cells were determined to be : for dsRNA , 200 micrograms/ml ; polyguacyl , 400 micrograms/ml ; tiloron , 100 micrograms/ml ; Tash-4 , 200 micrograms/ml , which corresponded to the antiproliferative effect of 200 units/ml of alpha-interferon and 40 units/ml of gamma-interferon .
	manualset3
250447	10	425578	7	NULL	NULL	0	NULL	400 micrograms/ml	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of the inducers producing death of 48-66 % of Raji cells were determined to be : for dsRNA , 200 micrograms/ml ; polyguacyl , 400 micrograms/ml ; tiloron , 100 micrograms/ml ; Tash-4 , 200 micrograms/ml , which corresponded to the antiproliferative effect of 200 units/ml of alpha-interferon and 40 units/ml of gamma-interferon .
	manualset3
250448	11	425578	7	NULL	NULL	0	NULL	tiloron	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of the inducers producing death of 48-66 % of Raji cells were determined to be : for dsRNA , 200 micrograms/ml ; polyguacyl , 400 micrograms/ml ; tiloron , 100 micrograms/ml ; Tash-4 , 200 micrograms/ml , which corresponded to the antiproliferative effect of 200 units/ml of alpha-interferon and 40 units/ml of gamma-interferon .
	manualset3
250449	12	425578	7	NULL	NULL	0	NULL	100 micrograms/ml	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of the inducers producing death of 48-66 % of Raji cells were determined to be : for dsRNA , 200 micrograms/ml ; polyguacyl , 400 micrograms/ml ; tiloron , 100 micrograms/ml ; Tash-4 , 200 micrograms/ml , which corresponded to the antiproliferative effect of 200 units/ml of alpha-interferon and 40 units/ml of gamma-interferon .
	manualset3
250450	13	425578	7	NULL	NULL	0	NULL	Tash-4	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of the inducers producing death of 48-66 % of Raji cells were determined to be : for dsRNA , 200 micrograms/ml ; polyguacyl , 400 micrograms/ml ; tiloron , 100 micrograms/ml ; Tash-4 , 200 micrograms/ml , which corresponded to the antiproliferative effect of 200 units/ml of alpha-interferon and 40 units/ml of gamma-interferon .
	manualset3
250451	14	425578	7	NULL	NULL	0	NULL	 200 micrograms/ml	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of the inducers producing death of 48-66 % of Raji cells were determined to be : for dsRNA , 200 micrograms/ml ; polyguacyl , 400 micrograms/ml ; tiloron , 100 micrograms/ml ; Tash-4 , 200 micrograms/ml , which corresponded to the antiproliferative effect of 200 units/ml of alpha-interferon and 40 units/ml of gamma-interferon .
	manualset3
250452	15	425578	7	NULL	NULL	0	NULL	antiproliferative effect 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of the inducers producing death of 48-66 % of Raji cells were determined to be : for dsRNA , 200 micrograms/ml ; polyguacyl , 400 micrograms/ml ; tiloron , 100 micrograms/ml ; Tash-4 , 200 micrograms/ml , which corresponded to the antiproliferative effect of 200 units/ml of alpha-interferon and 40 units/ml of gamma-interferon .
	manualset3
250453	16	425578	7	NULL	NULL	0	NULL	200 units/ml 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of the inducers producing death of 48-66 % of Raji cells were determined to be : for dsRNA , 200 micrograms/ml ; polyguacyl , 400 micrograms/ml ; tiloron , 100 micrograms/ml ; Tash-4 , 200 micrograms/ml , which corresponded to the antiproliferative effect of 200 units/ml of alpha-interferon and 40 units/ml of gamma-interferon .
	manualset3
250454	17	425578	7	NULL	NULL	0	NULL	alpha-interferon	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of the inducers producing death of 48-66 % of Raji cells were determined to be : for dsRNA , 200 micrograms/ml ; polyguacyl , 400 micrograms/ml ; tiloron , 100 micrograms/ml ; Tash-4 , 200 micrograms/ml , which corresponded to the antiproliferative effect of 200 units/ml of alpha-interferon and 40 units/ml of gamma-interferon .
	manualset3
250455	18	425578	7	NULL	NULL	0	NULL	40 units/ml	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of the inducers producing death of 48-66 % of Raji cells were determined to be : for dsRNA , 200 micrograms/ml ; polyguacyl , 400 micrograms/ml ; tiloron , 100 micrograms/ml ; Tash-4 , 200 micrograms/ml , which corresponded to the antiproliferative effect of 200 units/ml of alpha-interferon and 40 units/ml of gamma-interferon .
	manualset3
250456	19	425578	7	NULL	NULL	0	NULL	gamma-interferon	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Concentrations of the inducers producing death of 48-66 % of Raji cells were determined to be : for dsRNA , 200 micrograms/ml ; polyguacyl , 400 micrograms/ml ; tiloron , 100 micrograms/ml ; Tash-4 , 200 micrograms/ml , which corresponded to the antiproliferative effect of 200 units/ml of alpha-interferon and 40 units/ml of gamma-interferon .
	manualset3
250457	1	425579	7	NULL	NULL	0	NULL	ozone-depleting potential	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concern about the ozone-depleting potential of man-made chemicals has led the United Nations to control their usage .
	manualset3
250458	2	425579	7	NULL	NULL	0	NULL	man-made chemicals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Concern about the ozone-depleting potential of man-made chemicals has led the United Nations to control their usage .
	manualset3
250459	3	425579	7	NULL	NULL	0	NULL	United Nations	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Concern about the ozone-depleting potential of man-made chemicals has led the United Nations to control their usage .
	manualset3
250460	4	425579	7	NULL	NULL	0	NULL	usage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Concern about the ozone-depleting potential of man-made chemicals has led the United Nations to control their usage .
	manualset3
250461	1	425580	7	NULL	NULL	0	NULL	 fertility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Concern has been expressed regarding fertility following oral contraceptive ( OC ) use .
	manualset3
250462	2	425580	7	NULL	NULL	0	NULL	 oral contraceptive ( OC ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Concern has been expressed regarding fertility following oral contraceptive ( OC ) use .
	manualset3
252911	3	425580	7	NULL	NULL	0	NULL	concern	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Concern has been expressed regarding fertility following oral contraceptive ( OC ) use .
	manualset3
258753	4	425580	7	NULL	NULL	NULL	NULL	use	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Concern has been expressed regarding fertility following oral contraceptive ( OC ) use .
	manualset3
250465	1	425581	7	NULL	NULL	0	NULL	effectiveness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Concerning effectiveness , immobilisation , if necessary , should be restricted to certain patients and for short time periods .
	manualset3
250466	2	425581	7	NULL	NULL	0	NULL	 immobilisation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Concerning effectiveness , immobilisation , if necessary , should be restricted to certain patients and for short time periods .
	manualset3
250467	3	425581	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Concerning effectiveness , immobilisation , if necessary , should be restricted to certain patients and for short time periods .
	manualset3
250468	4	425581	7	NULL	NULL	0	NULL	short time periods	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Concerning effectiveness , immobilisation , if necessary , should be restricted to certain patients and for short time periods .
	manualset3
250469	1	425582	7	NULL	NULL	0	NULL	localisations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Concerning other localisations of atypical mycobacterial infections , iatrogenic causes seem to be increasing and cases of nosocomial transmissions have also been described .
	manualset3
250470	2	425582	7	NULL	NULL	0	NULL	atypical mycobacterial infections	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Concerning other localisations of atypical mycobacterial infections , iatrogenic causes seem to be increasing and cases of nosocomial transmissions have also been described .
	manualset3
250471	3	425582	7	NULL	NULL	0	NULL	 iatrogenic causes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Concerning other localisations of atypical mycobacterial infections , iatrogenic causes seem to be increasing and cases of nosocomial transmissions have also been described .
	manualset3
250472	4	425582	7	NULL	NULL	0	NULL	nosocomial transmissions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Concerning other localisations of atypical mycobacterial infections , iatrogenic causes seem to be increasing and cases of nosocomial transmissions have also been described .
	manualset3
250473	1	425583	7	NULL	NULL	0	NULL	LABORATORY DIAGNOSIS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( LABORATORY DIAGNOSIS OF INTESTINAL INFECTIONS IN THE DNEPROPETROVSK REGION ) .
	manualset3
250474	2	425583	7	NULL	NULL	0	NULL	INTESTINAL INFECTIONS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( LABORATORY DIAGNOSIS OF INTESTINAL INFECTIONS IN THE DNEPROPETROVSK REGION ) .
	manualset3
250475	3	425583	7	NULL	NULL	0	NULL	DNEPROPETROVSK REGION	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( LABORATORY DIAGNOSIS OF INTESTINAL INFECTIONS IN THE DNEPROPETROVSK REGION ) .
	manualset3
250476	1	425584	7	NULL	NULL	0	NULL	quality	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concerning the quality of the school report , the activity of the mother is more important than the activity of the father .
	manualset3
250477	2	425584	7	NULL	NULL	0	NULL	school report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Concerning the quality of the school report , the activity of the mother is more important than the activity of the father .
	manualset3
250478	3	425584	7	NULL	NULL	0	NULL	activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Concerning the quality of the school report , the activity of the mother is more important than the activity of the father .
	manualset3
250479	4	425584	7	NULL	NULL	0	NULL	mother	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Concerning the quality of the school report , the activity of the mother is more important than the activity of the father .
	manualset3
250480	5	425584	7	NULL	NULL	0	NULL	activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Concerning the quality of the school report , the activity of the mother is more important than the activity of the father .
	manualset3
250481	6	425584	7	NULL	NULL	0	NULL	 father	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Concerning the quality of the school report , the activity of the mother is more important than the activity of the father .
	manualset3
250482	1	425585	7	NULL	NULL	0	NULL	Conclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion : Our study brings evidence of a higher thrombophilic risk among the patients with early onset of the CVU as they had significantly higher prevalence of multiple ( 3 ) thrombophilias ( P = 0.03 ) , homozygous mutations ( P = 0.03 ) and family history of leg ulcer ( P = 0.02 ) when compared with patients with later onset .
	manualset3
250483	2	425585	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion : Our study brings evidence of a higher thrombophilic risk among the patients with early onset of the CVU as they had significantly higher prevalence of multiple ( 3 ) thrombophilias ( P = 0.03 ) , homozygous mutations ( P = 0.03 ) and family history of leg ulcer ( P = 0.02 ) when compared with patients with later onset .
	manualset3
250484	3	425585	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion : Our study brings evidence of a higher thrombophilic risk among the patients with early onset of the CVU as they had significantly higher prevalence of multiple ( 3 ) thrombophilias ( P = 0.03 ) , homozygous mutations ( P = 0.03 ) and family history of leg ulcer ( P = 0.02 ) when compared with patients with later onset .
	manualset3
250485	4	425585	7	NULL	NULL	0	NULL	thrombophilic risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion : Our study brings evidence of a higher thrombophilic risk among the patients with early onset of the CVU as they had significantly higher prevalence of multiple ( 3 ) thrombophilias ( P = 0.03 ) , homozygous mutations ( P = 0.03 ) and family history of leg ulcer ( P = 0.02 ) when compared with patients with later onset .
	manualset3
250486	5	425585	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion : Our study brings evidence of a higher thrombophilic risk among the patients with early onset of the CVU as they had significantly higher prevalence of multiple ( 3 ) thrombophilias ( P = 0.03 ) , homozygous mutations ( P = 0.03 ) and family history of leg ulcer ( P = 0.02 ) when compared with patients with later onset .
	manualset3
250487	6	425585	7	NULL	NULL	0	NULL	early onset	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion : Our study brings evidence of a higher thrombophilic risk among the patients with early onset of the CVU as they had significantly higher prevalence of multiple ( 3 ) thrombophilias ( P = 0.03 ) , homozygous mutations ( P = 0.03 ) and family history of leg ulcer ( P = 0.02 ) when compared with patients with later onset .
	manualset3
250488	7	425585	7	NULL	NULL	0	NULL	CVU	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion : Our study brings evidence of a higher thrombophilic risk among the patients with early onset of the CVU as they had significantly higher prevalence of multiple ( 3 ) thrombophilias ( P = 0.03 ) , homozygous mutations ( P = 0.03 ) and family history of leg ulcer ( P = 0.02 ) when compared with patients with later onset .
	manualset3
250489	8	425585	7	NULL	NULL	0	NULL	higher prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion : Our study brings evidence of a higher thrombophilic risk among the patients with early onset of the CVU as they had significantly higher prevalence of multiple ( 3 ) thrombophilias ( P = 0.03 ) , homozygous mutations ( P = 0.03 ) and family history of leg ulcer ( P = 0.02 ) when compared with patients with later onset .
	manualset3
250490	9	425585	7	NULL	NULL	0	NULL	multiple ( 3 ) thrombophilias 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion : Our study brings evidence of a higher thrombophilic risk among the patients with early onset of the CVU as they had significantly higher prevalence of multiple ( 3 ) thrombophilias ( P = 0.03 ) , homozygous mutations ( P = 0.03 ) and family history of leg ulcer ( P = 0.02 ) when compared with patients with later onset .
	manualset3
250491	10	425585	7	NULL	NULL	0	NULL	P = 0.03	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion : Our study brings evidence of a higher thrombophilic risk among the patients with early onset of the CVU as they had significantly higher prevalence of multiple ( 3 ) thrombophilias ( P = 0.03 ) , homozygous mutations ( P = 0.03 ) and family history of leg ulcer ( P = 0.02 ) when compared with patients with later onset .
	manualset3
250492	11	425585	7	NULL	NULL	0	NULL	 homozygous mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion : Our study brings evidence of a higher thrombophilic risk among the patients with early onset of the CVU as they had significantly higher prevalence of multiple ( 3 ) thrombophilias ( P = 0.03 ) , homozygous mutations ( P = 0.03 ) and family history of leg ulcer ( P = 0.02 ) when compared with patients with later onset .
	manualset3
250493	12	425585	7	NULL	NULL	NULL	NULL	P = 0.03	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Conclusion : Our study brings evidence of a higher thrombophilic risk among the patients with early onset of the CVU as they had significantly higher prevalence of multiple ( 3 ) thrombophilias ( P = 0.03 ) , homozygous mutations ( P = 0.03 ) and family history of leg ulcer ( P = 0.02 ) when compared with patients with later onset .
	manualset3
250494	13	425585	7	NULL	NULL	0	NULL	family history	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion : Our study brings evidence of a higher thrombophilic risk among the patients with early onset of the CVU as they had significantly higher prevalence of multiple ( 3 ) thrombophilias ( P = 0.03 ) , homozygous mutations ( P = 0.03 ) and family history of leg ulcer ( P = 0.02 ) when compared with patients with later onset .
	manualset3
250495	14	425585	7	NULL	NULL	0	NULL	leg ulcer	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion : Our study brings evidence of a higher thrombophilic risk among the patients with early onset of the CVU as they had significantly higher prevalence of multiple ( 3 ) thrombophilias ( P = 0.03 ) , homozygous mutations ( P = 0.03 ) and family history of leg ulcer ( P = 0.02 ) when compared with patients with later onset .
	manualset3
250496	15	425585	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion : Our study brings evidence of a higher thrombophilic risk among the patients with early onset of the CVU as they had significantly higher prevalence of multiple ( 3 ) thrombophilias ( P = 0.03 ) , homozygous mutations ( P = 0.03 ) and family history of leg ulcer ( P = 0.02 ) when compared with patients with later onset .
	manualset3
250497	16	425585	7	NULL	NULL	0	NULL	later onset	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion : Our study brings evidence of a higher thrombophilic risk among the patients with early onset of the CVU as they had significantly higher prevalence of multiple ( 3 ) thrombophilias ( P = 0.03 ) , homozygous mutations ( P = 0.03 ) and family history of leg ulcer ( P = 0.02 ) when compared with patients with later onset .
	manualset3
250498	17	425585	7	NULL	NULL	0	NULL	 P = 0.02	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion : Our study brings evidence of a higher thrombophilic risk among the patients with early onset of the CVU as they had significantly higher prevalence of multiple ( 3 ) thrombophilias ( P = 0.03 ) , homozygous mutations ( P = 0.03 ) and family history of leg ulcer ( P = 0.02 ) when compared with patients with later onset .
	manualset3
250508	1	425586	7	NULL	NULL	0	NULL	Conclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion : Decreased NHE activity in RBC after glucose-free HD is accompanied by decreased GSH concentration caused by lack of glucose in the dialysis fluid .
	manualset3
250509	2	425586	7	NULL	NULL	0	NULL	Decreased NHE activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion : Decreased NHE activity in RBC after glucose-free HD is accompanied by decreased GSH concentration caused by lack of glucose in the dialysis fluid .
	manualset3
250510	3	425586	7	NULL	NULL	0	NULL	RBC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion : Decreased NHE activity in RBC after glucose-free HD is accompanied by decreased GSH concentration caused by lack of glucose in the dialysis fluid .
	manualset3
250515	4	425586	7	NULL	NULL	0	NULL	glucose-free HD	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion : Decreased NHE activity in RBC after glucose-free HD is accompanied by decreased GSH concentration caused by lack of glucose in the dialysis fluid .
	manualset3
250517	5	425586	7	NULL	NULL	0	NULL	decreased GSH concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion : Decreased NHE activity in RBC after glucose-free HD is accompanied by decreased GSH concentration caused by lack of glucose in the dialysis fluid .
	manualset3
250519	6	425586	7	NULL	NULL	0	NULL	 glucose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion : Decreased NHE activity in RBC after glucose-free HD is accompanied by decreased GSH concentration caused by lack of glucose in the dialysis fluid .
	manualset3
250520	7	425586	7	NULL	NULL	0	NULL	dialysis fluid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion : Decreased NHE activity in RBC after glucose-free HD is accompanied by decreased GSH concentration caused by lack of glucose in the dialysis fluid .
	manualset3
250589	1	425588	7	NULL	NULL	0	NULL	Conclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion A QI approach , using learning networks to teach simple data-driven methods for addressing system failures , with increased training and resource inputs , can assist districts to quickly reach universal coverage targets .
	manualset3
250591	2	425588	7	NULL	NULL	0	NULL	QI approach	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion A QI approach , using learning networks to teach simple data-driven methods for addressing system failures , with increased training and resource inputs , can assist districts to quickly reach universal coverage targets .
	manualset3
250593	3	425588	7	NULL	NULL	0	NULL	 learning networks	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion A QI approach , using learning networks to teach simple data-driven methods for addressing system failures , with increased training and resource inputs , can assist districts to quickly reach universal coverage targets .
	manualset3
250595	4	425588	7	NULL	NULL	0	NULL	simple data-driven methods	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion A QI approach , using learning networks to teach simple data-driven methods for addressing system failures , with increased training and resource inputs , can assist districts to quickly reach universal coverage targets .
	manualset3
250597	5	425588	7	NULL	NULL	0	NULL	 system failures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion A QI approach , using learning networks to teach simple data-driven methods for addressing system failures , with increased training and resource inputs , can assist districts to quickly reach universal coverage targets .
	manualset3
250598	6	425588	7	NULL	NULL	0	NULL	training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion A QI approach , using learning networks to teach simple data-driven methods for addressing system failures , with increased training and resource inputs , can assist districts to quickly reach universal coverage targets .
	manualset3
250600	7	425588	7	NULL	NULL	0	NULL	 resource inputs 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion A QI approach , using learning networks to teach simple data-driven methods for addressing system failures , with increased training and resource inputs , can assist districts to quickly reach universal coverage targets .
	manualset3
250603	8	425588	7	NULL	NULL	0	NULL	 districts 	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion A QI approach , using learning networks to teach simple data-driven methods for addressing system failures , with increased training and resource inputs , can assist districts to quickly reach universal coverage targets .
	manualset3
250604	9	425588	7	NULL	NULL	0	NULL	universal coverage targets	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion A QI approach , using learning networks to teach simple data-driven methods for addressing system failures , with increased training and resource inputs , can assist districts to quickly reach universal coverage targets .
	manualset3
250613	1	425589	7	NULL	NULL	NULL	NULL	Conclusion 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Conclusion Drug treatment for LCOS in children with OHS across Europe is highly variable , possibly partly reflecting the lack of evidence and prescribing standards on the use of medicines .
	manualset3
250616	2	425589	7	NULL	NULL	0	NULL	Drug treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion Drug treatment for LCOS in children with OHS across Europe is highly variable , possibly partly reflecting the lack of evidence and prescribing standards on the use of medicines .
	manualset3
250619	3	425589	7	NULL	NULL	0	NULL	LCOS	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion Drug treatment for LCOS in children with OHS across Europe is highly variable , possibly partly reflecting the lack of evidence and prescribing standards on the use of medicines .
	manualset3
250621	4	425589	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion Drug treatment for LCOS in children with OHS across Europe is highly variable , possibly partly reflecting the lack of evidence and prescribing standards on the use of medicines .
	manualset3
250622	5	425589	7	NULL	NULL	0	NULL	OHS	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion Drug treatment for LCOS in children with OHS across Europe is highly variable , possibly partly reflecting the lack of evidence and prescribing standards on the use of medicines .
	manualset3
250623	6	425589	7	NULL	NULL	0	NULL	Europe	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion Drug treatment for LCOS in children with OHS across Europe is highly variable , possibly partly reflecting the lack of evidence and prescribing standards on the use of medicines .
	manualset3
250624	7	425589	7	NULL	NULL	0	NULL	lack	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion Drug treatment for LCOS in children with OHS across Europe is highly variable , possibly partly reflecting the lack of evidence and prescribing standards on the use of medicines .
	manualset3
250625	8	425589	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion Drug treatment for LCOS in children with OHS across Europe is highly variable , possibly partly reflecting the lack of evidence and prescribing standards on the use of medicines .
	manualset3
250626	9	425589	7	NULL	NULL	0	NULL	standards	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion Drug treatment for LCOS in children with OHS across Europe is highly variable , possibly partly reflecting the lack of evidence and prescribing standards on the use of medicines .
	manualset3
250627	10	425589	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion Drug treatment for LCOS in children with OHS across Europe is highly variable , possibly partly reflecting the lack of evidence and prescribing standards on the use of medicines .
	manualset3
250628	11	425589	7	NULL	NULL	0	NULL	medicines	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion Drug treatment for LCOS in children with OHS across Europe is highly variable , possibly partly reflecting the lack of evidence and prescribing standards on the use of medicines .
	manualset3
250629	1	425590	7	NULL	NULL	0	NULL	Conclusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion The Tuebingen CD-25 is a feasible instrument to assess HRQoL in CD in a clinical and investigative setting and provides normative data for all age groups and genders .
	manualset3
250630	2	425590	7	NULL	NULL	0	NULL	Tuebingen CD-25	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion The Tuebingen CD-25 is a feasible instrument to assess HRQoL in CD in a clinical and investigative setting and provides normative data for all age groups and genders .
	manualset3
250631	3	425590	7	NULL	NULL	0	NULL	feasible instrument 	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion The Tuebingen CD-25 is a feasible instrument to assess HRQoL in CD in a clinical and investigative setting and provides normative data for all age groups and genders .
	manualset3
250632	4	425590	7	NULL	NULL	0	NULL	HRQoL	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion The Tuebingen CD-25 is a feasible instrument to assess HRQoL in CD in a clinical and investigative setting and provides normative data for all age groups and genders .
	manualset3
250633	5	425590	7	NULL	NULL	0	NULL	CD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion The Tuebingen CD-25 is a feasible instrument to assess HRQoL in CD in a clinical and investigative setting and provides normative data for all age groups and genders .
	manualset3
250634	6	425590	7	NULL	NULL	0	NULL	clinical setting	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion The Tuebingen CD-25 is a feasible instrument to assess HRQoL in CD in a clinical and investigative setting and provides normative data for all age groups and genders .
	manualset3
250635	7	425590	7	NULL	NULL	0	NULL	investigative setting	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion The Tuebingen CD-25 is a feasible instrument to assess HRQoL in CD in a clinical and investigative setting and provides normative data for all age groups and genders .
	manualset3
250636	8	425590	7	NULL	NULL	0	NULL	normative data	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion The Tuebingen CD-25 is a feasible instrument to assess HRQoL in CD in a clinical and investigative setting and provides normative data for all age groups and genders .
	manualset3
250637	9	425590	7	NULL	NULL	0	NULL	age groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion The Tuebingen CD-25 is a feasible instrument to assess HRQoL in CD in a clinical and investigative setting and provides normative data for all age groups and genders .
	manualset3
250638	10	425590	7	NULL	NULL	0	NULL	genders	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusion The Tuebingen CD-25 is a feasible instrument to assess HRQoL in CD in a clinical and investigative setting and provides normative data for all age groups and genders .
	manualset3
250639	1	425591	7	NULL	NULL	0	NULL	Conclusions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : Our study establishes that calcification of the trochlea is common in the general population with a prevalence of 13 % .
	manualset3
250640	2	425591	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : Our study establishes that calcification of the trochlea is common in the general population with a prevalence of 13 % .
	manualset3
250641	3	425591	7	NULL	NULL	0	NULL	calcification 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : Our study establishes that calcification of the trochlea is common in the general population with a prevalence of 13 % .
	manualset3
250642	4	425591	7	NULL	NULL	0	NULL	 trochlea	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : Our study establishes that calcification of the trochlea is common in the general population with a prevalence of 13 % .
	manualset3
250643	5	425591	7	NULL	NULL	0	NULL	general population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : Our study establishes that calcification of the trochlea is common in the general population with a prevalence of 13 % .
	manualset3
250644	6	425591	7	NULL	NULL	0	NULL	 prevalence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : Our study establishes that calcification of the trochlea is common in the general population with a prevalence of 13 % .
	manualset3
250645	7	425591	7	NULL	NULL	0	NULL	13 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : Our study establishes that calcification of the trochlea is common in the general population with a prevalence of 13 % .
	manualset3
250646	1	425592	7	NULL	NULL	0	NULL	specialized anatomical museum 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( A specialized anatomical museum as a means of integration of the knowledge of the central nervous system and sense organs ) .
	manualset3
250647	2	425592	7	NULL	NULL	0	NULL	integration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( A specialized anatomical museum as a means of integration of the knowledge of the central nervous system and sense organs ) .
	manualset3
250648	3	425592	7	NULL	NULL	0	NULL	knowledge	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( A specialized anatomical museum as a means of integration of the knowledge of the central nervous system and sense organs ) .
	manualset3
250649	4	425592	7	NULL	NULL	0	NULL	 central nervous system	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( A specialized anatomical museum as a means of integration of the knowledge of the central nervous system and sense organs ) .
	manualset3
250650	5	425592	7	NULL	NULL	0	NULL	 sense organs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( A specialized anatomical museum as a means of integration of the knowledge of the central nervous system and sense organs ) .
	manualset3
250651	1	425593	7	NULL	NULL	0	NULL	LOCATION	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( LOCATION OF DIENCEPHALIC STRUCTURES IN THE DOG BY LIPIODOL INJECTION INTO THE LATERAL VENTRICLE ) .
	manualset3
250652	2	425593	7	NULL	NULL	0	NULL	DIENCEPHALIC STRUCTURES	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( LOCATION OF DIENCEPHALIC STRUCTURES IN THE DOG BY LIPIODOL INJECTION INTO THE LATERAL VENTRICLE ) .
	manualset3
250653	3	425593	7	NULL	NULL	0	NULL	DOG	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( LOCATION OF DIENCEPHALIC STRUCTURES IN THE DOG BY LIPIODOL INJECTION INTO THE LATERAL VENTRICLE ) .
	manualset3
250654	4	425593	7	NULL	NULL	0	NULL	LIPIODOL INJECTION	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( LOCATION OF DIENCEPHALIC STRUCTURES IN THE DOG BY LIPIODOL INJECTION INTO THE LATERAL VENTRICLE ) .
	manualset3
250655	5	425593	7	NULL	NULL	0	NULL	LATERAL VENTRICLE	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( LOCATION OF DIENCEPHALIC STRUCTURES IN THE DOG BY LIPIODOL INJECTION INTO THE LATERAL VENTRICLE ) .
	manualset3
250656	1	425594	7	NULL	NULL	0	NULL	Conclusions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : Approximately 5 % of the patients with Graves ' disease develop moderate to severe GO , with a similar risk in women and men with Graves ' disease .
	manualset3
250657	2	425594	7	NULL	NULL	0	NULL	5 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : Approximately 5 % of the patients with Graves ' disease develop moderate to severe GO , with a similar risk in women and men with Graves ' disease .
	manualset3
250658	3	425594	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : Approximately 5 % of the patients with Graves ' disease develop moderate to severe GO , with a similar risk in women and men with Graves ' disease .
	manualset3
250659	4	425594	7	NULL	NULL	0	NULL	Graves ' disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : Approximately 5 % of the patients with Graves ' disease develop moderate to severe GO , with a similar risk in women and men with Graves ' disease .
	manualset3
250660	5	425594	7	NULL	NULL	0	NULL	severe GO	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : Approximately 5 % of the patients with Graves ' disease develop moderate to severe GO , with a similar risk in women and men with Graves ' disease .
	manualset3
250661	6	425594	7	NULL	NULL	0	NULL	 risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : Approximately 5 % of the patients with Graves ' disease develop moderate to severe GO , with a similar risk in women and men with Graves ' disease .
	manualset3
250662	7	425594	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : Approximately 5 % of the patients with Graves ' disease develop moderate to severe GO , with a similar risk in women and men with Graves ' disease .
	manualset3
250663	8	425594	7	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : Approximately 5 % of the patients with Graves ' disease develop moderate to severe GO , with a similar risk in women and men with Graves ' disease .
	manualset3
250664	9	425594	7	NULL	NULL	0	NULL	Graves ' disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : Approximately 5 % of the patients with Graves ' disease develop moderate to severe GO , with a similar risk in women and men with Graves ' disease .
	manualset3
250665	1	425595	7	NULL	NULL	0	NULL	Conclusions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : Circulating adiponectin is independently and inversely associated with the risk of thyroid cancer .
	manualset3
250666	2	425595	7	NULL	NULL	0	NULL	Circulating adiponectin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : Circulating adiponectin is independently and inversely associated with the risk of thyroid cancer .
	manualset3
250667	3	425595	7	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : Circulating adiponectin is independently and inversely associated with the risk of thyroid cancer .
	manualset3
250668	4	425595	7	NULL	NULL	0	NULL	 thyroid cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : Circulating adiponectin is independently and inversely associated with the risk of thyroid cancer .
	manualset3
250669	1	425596	7	NULL	NULL	0	NULL	Conclusions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : The addition a jejuna pouch to Roux-en-Y reconstruction provides better reservoir function , but does not influence the incidence of reflux esophagitis .
	manualset3
250670	2	425596	7	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : The addition a jejuna pouch to Roux-en-Y reconstruction provides better reservoir function , but does not influence the incidence of reflux esophagitis .
	manualset3
250671	3	425596	7	NULL	NULL	0	NULL	jejuna pouch	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : The addition a jejuna pouch to Roux-en-Y reconstruction provides better reservoir function , but does not influence the incidence of reflux esophagitis .
	manualset3
250672	4	425596	7	NULL	NULL	0	NULL	Roux-en-Y reconstruction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : The addition a jejuna pouch to Roux-en-Y reconstruction provides better reservoir function , but does not influence the incidence of reflux esophagitis .
	manualset3
250673	5	425596	7	NULL	NULL	0	NULL	reservoir function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : The addition a jejuna pouch to Roux-en-Y reconstruction provides better reservoir function , but does not influence the incidence of reflux esophagitis .
	manualset3
250674	6	425596	7	NULL	NULL	0	NULL	 incidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : The addition a jejuna pouch to Roux-en-Y reconstruction provides better reservoir function , but does not influence the incidence of reflux esophagitis .
	manualset3
250675	7	425596	7	NULL	NULL	0	NULL	reflux esophagitis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : The addition a jejuna pouch to Roux-en-Y reconstruction provides better reservoir function , but does not influence the incidence of reflux esophagitis .
	manualset3
250676	1	425597	7	NULL	NULL	0	NULL	Conclusions 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : The treatment planning results demonstrate that the proposed framework can produce IMRT plans equivalent to or better than conventional IMRT plans gated at exhale .
	manualset3
250677	2	425597	7	NULL	NULL	0	NULL	treatment planning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : The treatment planning results demonstrate that the proposed framework can produce IMRT plans equivalent to or better than conventional IMRT plans gated at exhale .
	manualset3
250678	3	425597	7	NULL	NULL	0	NULL	 proposed framework	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : The treatment planning results demonstrate that the proposed framework can produce IMRT plans equivalent to or better than conventional IMRT plans gated at exhale .
	manualset3
250679	4	425597	7	NULL	NULL	0	NULL	IMRT plans	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : The treatment planning results demonstrate that the proposed framework can produce IMRT plans equivalent to or better than conventional IMRT plans gated at exhale .
	manualset3
250680	5	425597	7	NULL	NULL	0	NULL	conventional IMRT plans	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : The treatment planning results demonstrate that the proposed framework can produce IMRT plans equivalent to or better than conventional IMRT plans gated at exhale .
	manualset3
250681	6	425597	7	NULL	NULL	0	NULL	exhale	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions : The treatment planning results demonstrate that the proposed framework can produce IMRT plans equivalent to or better than conventional IMRT plans gated at exhale .
	manualset3
250682	1	425598	7	NULL	NULL	0	NULL	Conclusions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions Earlier return to dialysis therapy in failed kidney transplant patients tends to correlate with worse dialysis survival especially among healthiest and younger patients and women .
	manualset3
250683	2	425598	7	NULL	NULL	0	NULL	dialysis therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions Earlier return to dialysis therapy in failed kidney transplant patients tends to correlate with worse dialysis survival especially among healthiest and younger patients and women .
	manualset3
250684	3	425598	7	NULL	NULL	0	NULL	failed kidney transplant patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions Earlier return to dialysis therapy in failed kidney transplant patients tends to correlate with worse dialysis survival especially among healthiest and younger patients and women .
	manualset3
250685	4	425598	7	NULL	NULL	0	NULL	 worse dialysis survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions Earlier return to dialysis therapy in failed kidney transplant patients tends to correlate with worse dialysis survival especially among healthiest and younger patients and women .
	manualset3
250686	5	425598	7	NULL	NULL	0	NULL	healthiest patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions Earlier return to dialysis therapy in failed kidney transplant patients tends to correlate with worse dialysis survival especially among healthiest and younger patients and women .
	manualset3
250687	6	425598	7	NULL	NULL	0	NULL	younger patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions Earlier return to dialysis therapy in failed kidney transplant patients tends to correlate with worse dialysis survival especially among healthiest and younger patients and women .
	manualset3
250688	7	425598	7	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions Earlier return to dialysis therapy in failed kidney transplant patients tends to correlate with worse dialysis survival especially among healthiest and younger patients and women .
	manualset3
250689	1	425599	7	NULL	NULL	0	NULL	Conclusions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions regarding timing an oral rabies vaccination campaign based upon occurrence of rabies-related mortalities could not be presented because of the lack of obvious rabies mortality .
	manualset3
250690	2	425599	7	NULL	NULL	0	NULL	 timing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions regarding timing an oral rabies vaccination campaign based upon occurrence of rabies-related mortalities could not be presented because of the lack of obvious rabies mortality .
	manualset3
250691	3	425599	7	NULL	NULL	0	NULL	oral rabies vaccination campaign	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions regarding timing an oral rabies vaccination campaign based upon occurrence of rabies-related mortalities could not be presented because of the lack of obvious rabies mortality .
	manualset3
250692	4	425599	7	NULL	NULL	0	NULL	occurrence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions regarding timing an oral rabies vaccination campaign based upon occurrence of rabies-related mortalities could not be presented because of the lack of obvious rabies mortality .
	manualset3
250693	5	425599	7	NULL	NULL	0	NULL	rabies-related mortalities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions regarding timing an oral rabies vaccination campaign based upon occurrence of rabies-related mortalities could not be presented because of the lack of obvious rabies mortality .
	manualset3
250694	6	425599	7	NULL	NULL	0	NULL	rabies mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusions regarding timing an oral rabies vaccination campaign based upon occurrence of rabies-related mortalities could not be presented because of the lack of obvious rabies mortality .
	manualset3
250695	1	425600	7	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusively , this study offers a hypothesis that plectin deficient might play an important role in the tumorigenesis of hepatocellular carcinoma .
	manualset3
250696	2	425600	7	NULL	NULL	0	NULL	 hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusively , this study offers a hypothesis that plectin deficient might play an important role in the tumorigenesis of hepatocellular carcinoma .
	manualset3
250697	3	425600	7	NULL	NULL	0	NULL	 plectin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusively , this study offers a hypothesis that plectin deficient might play an important role in the tumorigenesis of hepatocellular carcinoma .
	manualset3
250698	4	425600	7	NULL	NULL	0	NULL	 role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusively , this study offers a hypothesis that plectin deficient might play an important role in the tumorigenesis of hepatocellular carcinoma .
	manualset3
250699	5	425600	7	NULL	NULL	0	NULL	tumorigenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusively , this study offers a hypothesis that plectin deficient might play an important role in the tumorigenesis of hepatocellular carcinoma .
	manualset3
250700	6	425600	7	NULL	NULL	0	NULL	 hepatocellular carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Conclusively , this study offers a hypothesis that plectin deficient might play an important role in the tumorigenesis of hepatocellular carcinoma .
	manualset3
250701	1	425601	7	NULL	NULL	0	NULL	Concomitant inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitant inhibition of arterial superprecipitation and phosphorylation by perhexiline ( IC50 = 33 microM ) and cinnarizine ( IC50 = 60 microM ) was similar to W-7 ( IC50 = 35 microM ) , and was characterized by a rightward shift in the pCa superprecipitation and pCa-light chain phosphorylation relationships , depressed maximum activity and attenuation by 2 microM exogenous calmodulin .
	manualset3
250702	2	425601	7	NULL	NULL	0	NULL	arterial superprecipitation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitant inhibition of arterial superprecipitation and phosphorylation by perhexiline ( IC50 = 33 microM ) and cinnarizine ( IC50 = 60 microM ) was similar to W-7 ( IC50 = 35 microM ) , and was characterized by a rightward shift in the pCa superprecipitation and pCa-light chain phosphorylation relationships , depressed maximum activity and attenuation by 2 microM exogenous calmodulin .
	manualset3
250703	3	425601	7	NULL	NULL	0	NULL	phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitant inhibition of arterial superprecipitation and phosphorylation by perhexiline ( IC50 = 33 microM ) and cinnarizine ( IC50 = 60 microM ) was similar to W-7 ( IC50 = 35 microM ) , and was characterized by a rightward shift in the pCa superprecipitation and pCa-light chain phosphorylation relationships , depressed maximum activity and attenuation by 2 microM exogenous calmodulin .
	manualset3
250704	4	425601	7	NULL	NULL	0	NULL	 perhexiline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitant inhibition of arterial superprecipitation and phosphorylation by perhexiline ( IC50 = 33 microM ) and cinnarizine ( IC50 = 60 microM ) was similar to W-7 ( IC50 = 35 microM ) , and was characterized by a rightward shift in the pCa superprecipitation and pCa-light chain phosphorylation relationships , depressed maximum activity and attenuation by 2 microM exogenous calmodulin .
	manualset3
250705	5	425601	7	NULL	NULL	0	NULL	IC50 = 33 microM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitant inhibition of arterial superprecipitation and phosphorylation by perhexiline ( IC50 = 33 microM ) and cinnarizine ( IC50 = 60 microM ) was similar to W-7 ( IC50 = 35 microM ) , and was characterized by a rightward shift in the pCa superprecipitation and pCa-light chain phosphorylation relationships , depressed maximum activity and attenuation by 2 microM exogenous calmodulin .
	manualset3
250706	6	425601	7	NULL	NULL	0	NULL	cinnarizine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitant inhibition of arterial superprecipitation and phosphorylation by perhexiline ( IC50 = 33 microM ) and cinnarizine ( IC50 = 60 microM ) was similar to W-7 ( IC50 = 35 microM ) , and was characterized by a rightward shift in the pCa superprecipitation and pCa-light chain phosphorylation relationships , depressed maximum activity and attenuation by 2 microM exogenous calmodulin .
	manualset3
250707	7	425601	7	NULL	NULL	0	NULL	IC50 = 60 microM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitant inhibition of arterial superprecipitation and phosphorylation by perhexiline ( IC50 = 33 microM ) and cinnarizine ( IC50 = 60 microM ) was similar to W-7 ( IC50 = 35 microM ) , and was characterized by a rightward shift in the pCa superprecipitation and pCa-light chain phosphorylation relationships , depressed maximum activity and attenuation by 2 microM exogenous calmodulin .
	manualset3
250708	8	425601	7	NULL	NULL	0	NULL	 W-7	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitant inhibition of arterial superprecipitation and phosphorylation by perhexiline ( IC50 = 33 microM ) and cinnarizine ( IC50 = 60 microM ) was similar to W-7 ( IC50 = 35 microM ) , and was characterized by a rightward shift in the pCa superprecipitation and pCa-light chain phosphorylation relationships , depressed maximum activity and attenuation by 2 microM exogenous calmodulin .
	manualset3
250709	9	425601	7	NULL	NULL	0	NULL	IC50 = 35 microM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitant inhibition of arterial superprecipitation and phosphorylation by perhexiline ( IC50 = 33 microM ) and cinnarizine ( IC50 = 60 microM ) was similar to W-7 ( IC50 = 35 microM ) , and was characterized by a rightward shift in the pCa superprecipitation and pCa-light chain phosphorylation relationships , depressed maximum activity and attenuation by 2 microM exogenous calmodulin .
	manualset3
250710	10	425601	7	NULL	NULL	0	NULL	rightward shift 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitant inhibition of arterial superprecipitation and phosphorylation by perhexiline ( IC50 = 33 microM ) and cinnarizine ( IC50 = 60 microM ) was similar to W-7 ( IC50 = 35 microM ) , and was characterized by a rightward shift in the pCa superprecipitation and pCa-light chain phosphorylation relationships , depressed maximum activity and attenuation by 2 microM exogenous calmodulin .
	manualset3
250711	11	425601	7	NULL	NULL	0	NULL	pCa superprecipitation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitant inhibition of arterial superprecipitation and phosphorylation by perhexiline ( IC50 = 33 microM ) and cinnarizine ( IC50 = 60 microM ) was similar to W-7 ( IC50 = 35 microM ) , and was characterized by a rightward shift in the pCa superprecipitation and pCa-light chain phosphorylation relationships , depressed maximum activity and attenuation by 2 microM exogenous calmodulin .
	manualset3
250712	12	425601	7	NULL	NULL	0	NULL	 pCa-light chain phosphorylation relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitant inhibition of arterial superprecipitation and phosphorylation by perhexiline ( IC50 = 33 microM ) and cinnarizine ( IC50 = 60 microM ) was similar to W-7 ( IC50 = 35 microM ) , and was characterized by a rightward shift in the pCa superprecipitation and pCa-light chain phosphorylation relationships , depressed maximum activity and attenuation by 2 microM exogenous calmodulin .
	manualset3
250713	13	425601	7	NULL	NULL	0	NULL	maximum activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitant inhibition of arterial superprecipitation and phosphorylation by perhexiline ( IC50 = 33 microM ) and cinnarizine ( IC50 = 60 microM ) was similar to W-7 ( IC50 = 35 microM ) , and was characterized by a rightward shift in the pCa superprecipitation and pCa-light chain phosphorylation relationships , depressed maximum activity and attenuation by 2 microM exogenous calmodulin .
	manualset3
250714	14	425601	7	NULL	NULL	0	NULL	attenuation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitant inhibition of arterial superprecipitation and phosphorylation by perhexiline ( IC50 = 33 microM ) and cinnarizine ( IC50 = 60 microM ) was similar to W-7 ( IC50 = 35 microM ) , and was characterized by a rightward shift in the pCa superprecipitation and pCa-light chain phosphorylation relationships , depressed maximum activity and attenuation by 2 microM exogenous calmodulin .
	manualset3
250715	15	425601	7	NULL	NULL	0	NULL	 2 microM 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitant inhibition of arterial superprecipitation and phosphorylation by perhexiline ( IC50 = 33 microM ) and cinnarizine ( IC50 = 60 microM ) was similar to W-7 ( IC50 = 35 microM ) , and was characterized by a rightward shift in the pCa superprecipitation and pCa-light chain phosphorylation relationships , depressed maximum activity and attenuation by 2 microM exogenous calmodulin .
	manualset3
250716	16	425601	7	NULL	NULL	0	NULL	exogenous calmodulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitant inhibition of arterial superprecipitation and phosphorylation by perhexiline ( IC50 = 33 microM ) and cinnarizine ( IC50 = 60 microM ) was similar to W-7 ( IC50 = 35 microM ) , and was characterized by a rightward shift in the pCa superprecipitation and pCa-light chain phosphorylation relationships , depressed maximum activity and attenuation by 2 microM exogenous calmodulin .
	manualset3
250717	1	425602	7	NULL	NULL	0	NULL	Late kidney rejection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Late kidney rejection : influence of imbalance in prednisone and azathioprine dosages ) .
	manualset3
250718	2	425602	7	NULL	NULL	0	NULL	 imbalance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Late kidney rejection : influence of imbalance in prednisone and azathioprine dosages ) .
	manualset3
250719	3	425602	7	NULL	NULL	NULL	NULL	prednisone dosages	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Late kidney rejection : influence of imbalance in prednisone and azathioprine dosages ) .
	manualset3
250720	4	425602	7	NULL	NULL	NULL	NULL	azathioprine dosages 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Late kidney rejection : influence of imbalance in prednisone and azathioprine dosages ) .
	manualset3
250721	1	425603	7	NULL	NULL	0	NULL	oligodendrocyte differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitant with oligodendrocyte differentiation , Tnc antagonized the expression of the signaling adaptor and RNA-binding molecule Sam68 .
	manualset3
250722	2	425603	7	NULL	NULL	0	NULL	 Tnc	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitant with oligodendrocyte differentiation , Tnc antagonized the expression of the signaling adaptor and RNA-binding molecule Sam68 .
	manualset3
250723	3	425603	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitant with oligodendrocyte differentiation , Tnc antagonized the expression of the signaling adaptor and RNA-binding molecule Sam68 .
	manualset3
250724	4	425603	7	NULL	NULL	NULL	NULL	signaling adaptor molecule	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Concomitant with oligodendrocyte differentiation , Tnc antagonized the expression of the signaling adaptor and RNA-binding molecule Sam68 .
	manualset3
250725	5	425603	7	NULL	NULL	0	NULL	RNA-binding molecule Sam68	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitant with oligodendrocyte differentiation , Tnc antagonized the expression of the signaling adaptor and RNA-binding molecule Sam68 .
	manualset3
250726	1	425604	7	NULL	NULL	0	NULL	analgesic activities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitantly , analgesic and anticonvulsive activities could increase whereas anticholinergic and antihistaminergic activities are expected to decrease .
	manualset3
250727	2	425604	7	NULL	NULL	0	NULL	anticonvulsive activities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitantly , analgesic and anticonvulsive activities could increase whereas anticholinergic and antihistaminergic activities are expected to decrease .
	manualset3
250728	3	425604	7	NULL	NULL	0	NULL	anticholinergic activities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitantly , analgesic and anticonvulsive activities could increase whereas anticholinergic and antihistaminergic activities are expected to decrease .
	manualset3
250729	4	425604	7	NULL	NULL	0	NULL	antihistaminergic activities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitantly , analgesic and anticonvulsive activities could increase whereas anticholinergic and antihistaminergic activities are expected to decrease .
	manualset3
250730	1	425605	7	NULL	NULL	0	NULL	decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitantly a decrease of myocardial contractility leads to a compromised left ventricular function with marked increases in left ventricular enddiastolic pressure .
	manualset3
250731	2	425605	7	NULL	NULL	0	NULL	myocardial contractility	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitantly a decrease of myocardial contractility leads to a compromised left ventricular function with marked increases in left ventricular enddiastolic pressure .
	manualset3
250732	3	425605	7	NULL	NULL	0	NULL	left ventricular function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitantly a decrease of myocardial contractility leads to a compromised left ventricular function with marked increases in left ventricular enddiastolic pressure .
	manualset3
250733	4	425605	7	NULL	NULL	0	NULL	left ventricular enddiastolic pressure	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concomitantly a decrease of myocardial contractility leads to a compromised left ventricular function with marked increases in left ventricular enddiastolic pressure .
	manualset3
250734	1	425606	7	NULL	NULL	0	NULL	family members	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Concordance in perceived needs of family members and care providers may lead to greater need satisfaction and it is advocated that both the patient and the family ( rather than the patient alone ) be the focus of treatment because of the relationship between social support and patient recovery .
	manualset3
250735	2	425606	7	NULL	NULL	0	NULL	care providers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Concordance in perceived needs of family members and care providers may lead to greater need satisfaction and it is advocated that both the patient and the family ( rather than the patient alone ) be the focus of treatment because of the relationship between social support and patient recovery .
	manualset3
250736	3	425606	7	NULL	NULL	NULL	NULL	satisfaction	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Concordance in perceived needs of family members and care providers may lead to greater need satisfaction and it is advocated that both the patient and the family ( rather than the patient alone ) be the focus of treatment because of the relationship between social support and patient recovery .
	manualset3
250737	4	425606	7	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Concordance in perceived needs of family members and care providers may lead to greater need satisfaction and it is advocated that both the patient and the family ( rather than the patient alone ) be the focus of treatment because of the relationship between social support and patient recovery .
	manualset3
250738	5	425606	7	NULL	NULL	0	NULL	 family	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Concordance in perceived needs of family members and care providers may lead to greater need satisfaction and it is advocated that both the patient and the family ( rather than the patient alone ) be the focus of treatment because of the relationship between social support and patient recovery .
	manualset3
250739	6	425606	7	NULL	NULL	0	NULL	patient 	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Concordance in perceived needs of family members and care providers may lead to greater need satisfaction and it is advocated that both the patient and the family ( rather than the patient alone ) be the focus of treatment because of the relationship between social support and patient recovery .
	manualset3
250740	7	425606	7	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Concordance in perceived needs of family members and care providers may lead to greater need satisfaction and it is advocated that both the patient and the family ( rather than the patient alone ) be the focus of treatment because of the relationship between social support and patient recovery .
	manualset3
250741	8	425606	7	NULL	NULL	0	NULL	 relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Concordance in perceived needs of family members and care providers may lead to greater need satisfaction and it is advocated that both the patient and the family ( rather than the patient alone ) be the focus of treatment because of the relationship between social support and patient recovery .
	manualset3
250742	9	425606	7	NULL	NULL	0	NULL	social support 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Concordance in perceived needs of family members and care providers may lead to greater need satisfaction and it is advocated that both the patient and the family ( rather than the patient alone ) be the focus of treatment because of the relationship between social support and patient recovery .
	manualset3
250743	10	425606	7	NULL	NULL	0	NULL	patient recovery	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Concordance in perceived needs of family members and care providers may lead to greater need satisfaction and it is advocated that both the patient and the family ( rather than the patient alone ) be the focus of treatment because of the relationship between social support and patient recovery .
	manualset3
252918	11	425606	7	NULL	NULL	0	NULL	Concordance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Concordance in perceived needs of family members and care providers may lead to greater need satisfaction and it is advocated that both the patient and the family ( rather than the patient alone ) be the focus of treatment because of the relationship between social support and patient recovery .
	manualset3
252919	12	425606	7	NULL	NULL	0	NULL	perceived needs	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Concordance in perceived needs of family members and care providers may lead to greater need satisfaction and it is advocated that both the patient and the family ( rather than the patient alone ) be the focus of treatment because of the relationship between social support and patient recovery .
	manualset3
250744	1	425607	7	NULL	NULL	0	NULL	smooth pursuit	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Concordance of smooth pursuit and saccadic measures in normal monozygotic twin pairs .
	manualset3
250745	2	425607	7	NULL	NULL	0	NULL	saccadic measures	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Concordance of smooth pursuit and saccadic measures in normal monozygotic twin pairs .
	manualset3
250746	3	425607	7	NULL	NULL	0	NULL	normal monozygotic twin pairs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Concordance of smooth pursuit and saccadic measures in normal monozygotic twin pairs .
	manualset3
252920	4	425607	7	NULL	NULL	0	NULL	Concordance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Concordance of smooth pursuit and saccadic measures in normal monozygotic twin pairs .
	manualset3
250747	1	425608	7	NULL	NULL	0	NULL	 intra-class correlation coefficient	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Concordance was measured by the intra-class correlation coefficient of variation .
	manualset3
250748	2	425608	7	NULL	NULL	0	NULL	variation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Concordance was measured by the intra-class correlation coefficient of variation .
	manualset3
252921	3	425608	7	NULL	NULL	0	NULL	Concordance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Concordance was measured by the intra-class correlation coefficient of variation .
	manualset3
250758	1	425609	7	NULL	NULL	0	NULL	Concurrent administration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Concurrent administration of aqueous Azadirachta indica ( neem ) leaf extract with DOCA-salt prevents the development of hypertension and accompanying electrocardiogram changes in the rat .
	manualset3
250761	2	425609	7	NULL	NULL	0	NULL	aqueous Azadirachta indica ( neem ) leaf extract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Concurrent administration of aqueous Azadirachta indica ( neem ) leaf extract with DOCA-salt prevents the development of hypertension and accompanying electrocardiogram changes in the rat .
	manualset3
250763	3	425609	7	NULL	NULL	0	NULL	 DOCA-salt	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Concurrent administration of aqueous Azadirachta indica ( neem ) leaf extract with DOCA-salt prevents the development of hypertension and accompanying electrocardiogram changes in the rat .
	manualset3
250764	4	425609	7	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Concurrent administration of aqueous Azadirachta indica ( neem ) leaf extract with DOCA-salt prevents the development of hypertension and accompanying electrocardiogram changes in the rat .
	manualset3
250766	5	425609	7	NULL	NULL	0	NULL	hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Concurrent administration of aqueous Azadirachta indica ( neem ) leaf extract with DOCA-salt prevents the development of hypertension and accompanying electrocardiogram changes in the rat .
	manualset3
250771	6	425609	7	NULL	NULL	0	NULL	electrocardiogram changes 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Concurrent administration of aqueous Azadirachta indica ( neem ) leaf extract with DOCA-salt prevents the development of hypertension and accompanying electrocardiogram changes in the rat .
	manualset3
250772	7	425609	7	NULL	NULL	0	NULL	rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Concurrent administration of aqueous Azadirachta indica ( neem ) leaf extract with DOCA-salt prevents the development of hypertension and accompanying electrocardiogram changes in the rat .
	manualset3
250774	1	425610	7	NULL	NULL	0	NULL	Left ventricular function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Left ventricular function in aortic and mitral insufficiency studied with digitalized echocardiograms and apex cardiograms ) .
	manualset3
250776	2	425610	7	NULL	NULL	0	NULL	aortic  insufficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Left ventricular function in aortic and mitral insufficiency studied with digitalized echocardiograms and apex cardiograms ) .
	manualset3
250777	3	425610	7	NULL	NULL	0	NULL	mitral insufficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Left ventricular function in aortic and mitral insufficiency studied with digitalized echocardiograms and apex cardiograms ) .
	manualset3
250778	4	425610	7	NULL	NULL	0	NULL	digitalized echocardiograms	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Left ventricular function in aortic and mitral insufficiency studied with digitalized echocardiograms and apex cardiograms ) .
	manualset3
250781	5	425610	7	NULL	NULL	0	NULL	apex cardiograms	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Left ventricular function in aortic and mitral insufficiency studied with digitalized echocardiograms and apex cardiograms ) .
	manualset3
250798	1	425611	7	NULL	NULL	0	NULL	mean ( pooled ) serum leptin concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concurrently , mean ( pooled ) serum leptin concentrations fell by 75 % ( P = 0.0003 ) , and insulin-like growth factor I ( IGF-I ; P & lt ; 0.05 ) and insulin decreased significantly ( P = 0.0018 ) .
	manualset3
250799	2	425611	7	NULL	NULL	0	NULL	 75 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concurrently , mean ( pooled ) serum leptin concentrations fell by 75 % ( P = 0.0003 ) , and insulin-like growth factor I ( IGF-I ; P & lt ; 0.05 ) and insulin decreased significantly ( P = 0.0018 ) .
	manualset3
250800	3	425611	7	NULL	NULL	0	NULL	P = 0.0003	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concurrently , mean ( pooled ) serum leptin concentrations fell by 75 % ( P = 0.0003 ) , and insulin-like growth factor I ( IGF-I ; P & lt ; 0.05 ) and insulin decreased significantly ( P = 0.0018 ) .
	manualset3
250801	4	425611	7	NULL	NULL	0	NULL	insulin-like growth factor I 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Concurrently , mean ( pooled ) serum leptin concentrations fell by 75 % ( P = 0.0003 ) , and insulin-like growth factor I ( IGF-I ; P & lt ; 0.05 ) and insulin decreased significantly ( P = 0.0018 ) .
	manualset3
250802	5	425611	7	NULL	NULL	0	NULL	IGF-I	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Concurrently , mean ( pooled ) serum leptin concentrations fell by 75 % ( P = 0.0003 ) , and insulin-like growth factor I ( IGF-I ; P & lt ; 0.05 ) and insulin decreased significantly ( P = 0.0018 ) .
	manualset3
250803	6	425611	7	NULL	NULL	0	NULL	 P & lt ; 0.05	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concurrently , mean ( pooled ) serum leptin concentrations fell by 75 % ( P = 0.0003 ) , and insulin-like growth factor I ( IGF-I ; P & lt ; 0.05 ) and insulin decreased significantly ( P = 0.0018 ) .
	manualset3
250804	7	425611	7	NULL	NULL	0	NULL	insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Concurrently , mean ( pooled ) serum leptin concentrations fell by 75 % ( P = 0.0003 ) , and insulin-like growth factor I ( IGF-I ; P & lt ; 0.05 ) and insulin decreased significantly ( P = 0.0018 ) .
	manualset3
250805	8	425611	7	NULL	NULL	0	NULL	P = 0.0018	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Concurrently , mean ( pooled ) serum leptin concentrations fell by 75 % ( P = 0.0003 ) , and insulin-like growth factor I ( IGF-I ; P & lt ; 0.05 ) and insulin decreased significantly ( P = 0.0018 ) .
	manualset3
250806	1	425612	7	NULL	NULL	0	NULL	selective expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Concurrently , the selective expression of cell adhesion molecules on different organs and endothelia , in conjunction with the presence of dissimilar adhesion ligands on various colorectal cancer cell lines , suggest that CAMs may also mediate the selection of the host organ , for the development of distant colorectal metastases .
	manualset3
250807	2	425612	7	NULL	NULL	0	NULL	cell adhesion molecules	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Concurrently , the selective expression of cell adhesion molecules on different organs and endothelia , in conjunction with the presence of dissimilar adhesion ligands on various colorectal cancer cell lines , suggest that CAMs may also mediate the selection of the host organ , for the development of distant colorectal metastases .
	manualset3
250808	3	425612	7	NULL	NULL	0	NULL	different organs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Concurrently , the selective expression of cell adhesion molecules on different organs and endothelia , in conjunction with the presence of dissimilar adhesion ligands on various colorectal cancer cell lines , suggest that CAMs may also mediate the selection of the host organ , for the development of distant colorectal metastases .
	manualset3
250809	4	425612	7	NULL	NULL	0	NULL	endothelia	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Concurrently , the selective expression of cell adhesion molecules on different organs and endothelia , in conjunction with the presence of dissimilar adhesion ligands on various colorectal cancer cell lines , suggest that CAMs may also mediate the selection of the host organ , for the development of distant colorectal metastases .
	manualset3
250811	5	425612	7	NULL	NULL	0	NULL	conjunction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Concurrently , the selective expression of cell adhesion molecules on different organs and endothelia , in conjunction with the presence of dissimilar adhesion ligands on various colorectal cancer cell lines , suggest that CAMs may also mediate the selection of the host organ , for the development of distant colorectal metastases .
	manualset3
250812	6	425612	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Concurrently , the selective expression of cell adhesion molecules on different organs and endothelia , in conjunction with the presence of dissimilar adhesion ligands on various colorectal cancer cell lines , suggest that CAMs may also mediate the selection of the host organ , for the development of distant colorectal metastases .
	manualset3
250813	7	425612	7	NULL	NULL	0	NULL	dissimilar adhesion ligands	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Concurrently , the selective expression of cell adhesion molecules on different organs and endothelia , in conjunction with the presence of dissimilar adhesion ligands on various colorectal cancer cell lines , suggest that CAMs may also mediate the selection of the host organ , for the development of distant colorectal metastases .
	manualset3
250814	8	425612	7	NULL	NULL	0	NULL	colorectal cancer cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Concurrently , the selective expression of cell adhesion molecules on different organs and endothelia , in conjunction with the presence of dissimilar adhesion ligands on various colorectal cancer cell lines , suggest that CAMs may also mediate the selection of the host organ , for the development of distant colorectal metastases .
	manualset3
250815	9	425612	7	NULL	NULL	0	NULL	CAMs	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Concurrently , the selective expression of cell adhesion molecules on different organs and endothelia , in conjunction with the presence of dissimilar adhesion ligands on various colorectal cancer cell lines , suggest that CAMs may also mediate the selection of the host organ , for the development of distant colorectal metastases .
	manualset3
250816	10	425612	7	NULL	NULL	0	NULL	selection 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Concurrently , the selective expression of cell adhesion molecules on different organs and endothelia , in conjunction with the presence of dissimilar adhesion ligands on various colorectal cancer cell lines , suggest that CAMs may also mediate the selection of the host organ , for the development of distant colorectal metastases .
	manualset3
250817	11	425612	7	NULL	NULL	0	NULL	host organ	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Concurrently , the selective expression of cell adhesion molecules on different organs and endothelia , in conjunction with the presence of dissimilar adhesion ligands on various colorectal cancer cell lines , suggest that CAMs may also mediate the selection of the host organ , for the development of distant colorectal metastases .
	manualset3
250818	12	425612	7	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Concurrently , the selective expression of cell adhesion molecules on different organs and endothelia , in conjunction with the presence of dissimilar adhesion ligands on various colorectal cancer cell lines , suggest that CAMs may also mediate the selection of the host organ , for the development of distant colorectal metastases .
	manualset3
250819	13	425612	7	NULL	NULL	0	NULL	distant colorectal metastases	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Concurrently , the selective expression of cell adhesion molecules on different organs and endothelia , in conjunction with the presence of dissimilar adhesion ligands on various colorectal cancer cell lines , suggest that CAMs may also mediate the selection of the host organ , for the development of distant colorectal metastases .
	manualset3
250820	1	425613	7	NULL	NULL	0	NULL	Conditional deletion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Conditional deletion of Dscam reproduces cell spacing , cell number and dendrite arborization defects .
	manualset3
250821	2	425613	7	NULL	NULL	0	NULL	Dscam	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Conditional deletion of Dscam reproduces cell spacing , cell number and dendrite arborization defects .
	manualset3
250822	3	425613	7	NULL	NULL	0	NULL	cell spacing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Conditional deletion of Dscam reproduces cell spacing , cell number and dendrite arborization defects .
	manualset3
250823	4	425613	7	NULL	NULL	0	NULL	cell number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Conditional deletion of Dscam reproduces cell spacing , cell number and dendrite arborization defects .
	manualset3
250824	5	425613	7	NULL	NULL	0	NULL	dendrite arborization defects 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conditional deletion of Dscam reproduces cell spacing , cell number and dendrite arborization defects .
	manualset3
250825	1	425614	7	NULL	NULL	0	NULL	Conditional depletion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Conditional depletion with diphtheria toxin of CD11b , but not CD11c cells , in oral tissues impairs CD4 T-cell priming in CLNs .
	manualset3
250826	2	425614	7	NULL	NULL	0	NULL	diphtheria toxin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Conditional depletion with diphtheria toxin of CD11b , but not CD11c cells , in oral tissues impairs CD4 T-cell priming in CLNs .
	manualset3
250827	3	425614	7	NULL	NULL	0	NULL	CD11b	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Conditional depletion with diphtheria toxin of CD11b , but not CD11c cells , in oral tissues impairs CD4 T-cell priming in CLNs .
	manualset3
250828	4	425614	7	NULL	NULL	0	NULL	CD11c cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Conditional depletion with diphtheria toxin of CD11b , but not CD11c cells , in oral tissues impairs CD4 T-cell priming in CLNs .
	manualset3
250829	5	425614	7	NULL	NULL	0	NULL	oral tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Conditional depletion with diphtheria toxin of CD11b , but not CD11c cells , in oral tissues impairs CD4 T-cell priming in CLNs .
	manualset3
250830	6	425614	7	NULL	NULL	0	NULL	CD4 T-cell priming 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Conditional depletion with diphtheria toxin of CD11b , but not CD11c cells , in oral tissues impairs CD4 T-cell priming in CLNs .
	manualset3
250831	7	425614	7	NULL	NULL	0	NULL	CLNs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Conditional depletion with diphtheria toxin of CD11b , but not CD11c cells , in oral tissues impairs CD4 T-cell priming in CLNs .
	manualset3
250832	1	425615	7	NULL	NULL	0	NULL	Conditioned media	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Conditioned media collected from tissue slices containing the axotomized central nervous system neurons exhibit BDCF activity .
	manualset3
250833	2	425615	7	NULL	NULL	0	NULL	tissue slices	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Conditioned media collected from tissue slices containing the axotomized central nervous system neurons exhibit BDCF activity .
	manualset3
250834	3	425615	7	NULL	NULL	0	NULL	 axotomized central nervous system neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Conditioned media collected from tissue slices containing the axotomized central nervous system neurons exhibit BDCF activity .
	manualset3
250835	4	425615	7	NULL	NULL	0	NULL	BDCF activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Conditioned media collected from tissue slices containing the axotomized central nervous system neurons exhibit BDCF activity .
	manualset3
250836	1	425616	7	NULL	NULL	0	NULL	Conditioned asthma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conditioned asthma in guinea pigs .
	manualset3
250837	2	425616	7	NULL	NULL	0	NULL	guinea pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Conditioned asthma in guinea pigs .
	manualset3
250838	1	425617	7	NULL	NULL	0	NULL	Conditions	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Conditions with increased cyclic AMP were associated with a stimulated efflux of 45Ca from the secretory granules but not from the mitochondria .
	manualset3
250839	2	425617	7	NULL	NULL	0	NULL	cyclic AMP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Conditions with increased cyclic AMP were associated with a stimulated efflux of 45Ca from the secretory granules but not from the mitochondria .
	manualset3
250840	3	425617	7	NULL	NULL	0	NULL	 stimulated efflux 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conditions with increased cyclic AMP were associated with a stimulated efflux of 45Ca from the secretory granules but not from the mitochondria .
	manualset3
250841	4	425617	7	NULL	NULL	0	NULL	45Ca	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Conditions with increased cyclic AMP were associated with a stimulated efflux of 45Ca from the secretory granules but not from the mitochondria .
	manualset3
250842	5	425617	7	NULL	NULL	0	NULL	 secretory granules 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Conditions with increased cyclic AMP were associated with a stimulated efflux of 45Ca from the secretory granules but not from the mitochondria .
	manualset3
250843	6	425617	7	NULL	NULL	0	NULL	mitochondria	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Conditions with increased cyclic AMP were associated with a stimulated efflux of 45Ca from the secretory granules but not from the mitochondria .
	manualset3
250844	1	425618	7	NULL	NULL	0	NULL	Cone beam CT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Cone beam CT of the mandibular ramus and body was performed in 10 randomly selected patients ( study group ) and the precise location of the IAN was determined preoperatively and intraoperatively .
	manualset3
250845	2	425618	7	NULL	NULL	0	NULL	mandibular ramus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Cone beam CT of the mandibular ramus and body was performed in 10 randomly selected patients ( study group ) and the precise location of the IAN was determined preoperatively and intraoperatively .
	manualset3
250846	3	425618	7	NULL	NULL	0	NULL	body	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Cone beam CT of the mandibular ramus and body was performed in 10 randomly selected patients ( study group ) and the precise location of the IAN was determined preoperatively and intraoperatively .
	manualset3
250847	4	425618	7	NULL	NULL	0	NULL	10 randomly selected patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Cone beam CT of the mandibular ramus and body was performed in 10 randomly selected patients ( study group ) and the precise location of the IAN was determined preoperatively and intraoperatively .
	manualset3
250848	5	425618	7	NULL	NULL	0	NULL	study group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Cone beam CT of the mandibular ramus and body was performed in 10 randomly selected patients ( study group ) and the precise location of the IAN was determined preoperatively and intraoperatively .
	manualset3
250849	6	425618	7	NULL	NULL	0	NULL	 precise location	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Cone beam CT of the mandibular ramus and body was performed in 10 randomly selected patients ( study group ) and the precise location of the IAN was determined preoperatively and intraoperatively .
	manualset3
250850	7	425618	7	NULL	NULL	0	NULL	IAN	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Cone beam CT of the mandibular ramus and body was performed in 10 randomly selected patients ( study group ) and the precise location of the IAN was determined preoperatively and intraoperatively .
	manualset3
250851	1	425619	7	NULL	NULL	0	NULL	Conferees	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Conferees were given news on the latest advances in the development of innovative antibiotics belonging to these increasingly important groups of drugs , and learned of their expanding clinical indications .
	manualset3
250852	2	425619	7	NULL	NULL	0	NULL	news 	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Conferees were given news on the latest advances in the development of innovative antibiotics belonging to these increasingly important groups of drugs , and learned of their expanding clinical indications .
	manualset3
250853	3	425619	7	NULL	NULL	0	NULL	latest advances	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conferees were given news on the latest advances in the development of innovative antibiotics belonging to these increasingly important groups of drugs , and learned of their expanding clinical indications .
	manualset3
250854	4	425619	7	NULL	NULL	0	NULL	development 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conferees were given news on the latest advances in the development of innovative antibiotics belonging to these increasingly important groups of drugs , and learned of their expanding clinical indications .
	manualset3
250855	5	425619	7	NULL	NULL	0	NULL	 innovative antibiotics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Conferees were given news on the latest advances in the development of innovative antibiotics belonging to these increasingly important groups of drugs , and learned of their expanding clinical indications .
	manualset3
250856	6	425619	7	NULL	NULL	0	NULL	important groups	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Conferees were given news on the latest advances in the development of innovative antibiotics belonging to these increasingly important groups of drugs , and learned of their expanding clinical indications .
	manualset3
250857	7	425619	7	NULL	NULL	0	NULL	drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Conferees were given news on the latest advances in the development of innovative antibiotics belonging to these increasingly important groups of drugs , and learned of their expanding clinical indications .
	manualset3
250858	8	425619	7	NULL	NULL	0	NULL	 clinical indications 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conferees were given news on the latest advances in the development of innovative antibiotics belonging to these increasingly important groups of drugs , and learned of their expanding clinical indications .
	manualset3
250862	1	425620	7	NULL	NULL	0	NULL	Lenin 's principle	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Lenin 's principle of party adherence and medicine ) .
	manualset3
250863	2	425620	7	NULL	NULL	0	NULL	party adherence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Lenin 's principle of party adherence and medicine ) .
	manualset3
250864	3	425620	7	NULL	NULL	0	NULL	medicine	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Lenin 's principle of party adherence and medicine ) .
	manualset3
250859	1	425621	7	NULL	NULL	0	NULL	Confirmation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Confirmation of E. bieneusi was done using transmission electron microscopy .
	manualset3
250860	2	425621	7	NULL	NULL	0	NULL	E. bieneusi	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Confirmation of E. bieneusi was done using transmission electron microscopy .
	manualset3
250861	3	425621	7	NULL	NULL	0	NULL	transmission electron microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Confirmation of E. bieneusi was done using transmission electron microscopy .
	manualset3
250865	1	425622	7	NULL	NULL	0	NULL	Confirmation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Confirmation of these findings in other patients would help elucidating mechanisms of synaptic dysfunction in this disease , and highlight the role of A in both early and late periods of life .
	manualset3
250866	2	425622	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Confirmation of these findings in other patients would help elucidating mechanisms of synaptic dysfunction in this disease , and highlight the role of A in both early and late periods of life .
	manualset3
250867	3	425622	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Confirmation of these findings in other patients would help elucidating mechanisms of synaptic dysfunction in this disease , and highlight the role of A in both early and late periods of life .
	manualset3
250868	4	425622	7	NULL	NULL	0	NULL	mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Confirmation of these findings in other patients would help elucidating mechanisms of synaptic dysfunction in this disease , and highlight the role of A in both early and late periods of life .
	manualset3
250869	5	425622	7	NULL	NULL	0	NULL	synaptic dysfunction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Confirmation of these findings in other patients would help elucidating mechanisms of synaptic dysfunction in this disease , and highlight the role of A in both early and late periods of life .
	manualset3
250870	6	425622	7	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Confirmation of these findings in other patients would help elucidating mechanisms of synaptic dysfunction in this disease , and highlight the role of A in both early and late periods of life .
	manualset3
250871	7	425622	7	NULL	NULL	0	NULL	role	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Confirmation of these findings in other patients would help elucidating mechanisms of synaptic dysfunction in this disease , and highlight the role of A in both early and late periods of life .
	manualset3
250872	8	425622	7	NULL	NULL	0	NULL	 A	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Confirmation of these findings in other patients would help elucidating mechanisms of synaptic dysfunction in this disease , and highlight the role of A in both early and late periods of life .
	manualset3
250873	9	425622	7	NULL	NULL	0	NULL	early periods	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Confirmation of these findings in other patients would help elucidating mechanisms of synaptic dysfunction in this disease , and highlight the role of A in both early and late periods of life .
	manualset3
250874	10	425622	7	NULL	NULL	0	NULL	 late periods	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Confirmation of these findings in other patients would help elucidating mechanisms of synaptic dysfunction in this disease , and highlight the role of A in both early and late periods of life .
	manualset3
250875	11	425622	7	NULL	NULL	0	NULL	life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Confirmation of these findings in other patients would help elucidating mechanisms of synaptic dysfunction in this disease , and highlight the role of A in both early and late periods of life .
	manualset3
250876	1	425623	7	NULL	NULL	0	NULL	Confirmation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Confirmation of these results was the observation that the high density , small , resting B-cells had negligible background proliferation and immunoglobulin secretion , while the low density , larger , activated B-cells had marked background proliferative and antibody responses .
	manualset3
250877	2	425623	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Confirmation of these results was the observation that the high density , small , resting B-cells had negligible background proliferation and immunoglobulin secretion , while the low density , larger , activated B-cells had marked background proliferative and antibody responses .
	manualset3
250878	3	425623	7	NULL	NULL	0	NULL	observation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Confirmation of these results was the observation that the high density , small , resting B-cells had negligible background proliferation and immunoglobulin secretion , while the low density , larger , activated B-cells had marked background proliferative and antibody responses .
	manualset3
250879	4	425623	7	NULL	NULL	0	NULL	high density	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Confirmation of these results was the observation that the high density , small , resting B-cells had negligible background proliferation and immunoglobulin secretion , while the low density , larger , activated B-cells had marked background proliferative and antibody responses .
	manualset3
250880	5	425623	7	NULL	NULL	0	NULL	small , resting B-cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Confirmation of these results was the observation that the high density , small , resting B-cells had negligible background proliferation and immunoglobulin secretion , while the low density , larger , activated B-cells had marked background proliferative and antibody responses .
	manualset3
250881	6	425623	7	NULL	NULL	0	NULL	background proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Confirmation of these results was the observation that the high density , small , resting B-cells had negligible background proliferation and immunoglobulin secretion , while the low density , larger , activated B-cells had marked background proliferative and antibody responses .
	manualset3
250882	7	425623	7	NULL	NULL	0	NULL	immunoglobulin secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Confirmation of these results was the observation that the high density , small , resting B-cells had negligible background proliferation and immunoglobulin secretion , while the low density , larger , activated B-cells had marked background proliferative and antibody responses .
	manualset3
250883	8	425623	7	NULL	NULL	0	NULL	low density	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Confirmation of these results was the observation that the high density , small , resting B-cells had negligible background proliferation and immunoglobulin secretion , while the low density , larger , activated B-cells had marked background proliferative and antibody responses .
	manualset3
250884	9	425623	7	NULL	NULL	0	NULL	 activated B-cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Confirmation of these results was the observation that the high density , small , resting B-cells had negligible background proliferation and immunoglobulin secretion , while the low density , larger , activated B-cells had marked background proliferative and antibody responses .
	manualset3
250885	10	425623	7	NULL	NULL	0	NULL	background proliferative responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Confirmation of these results was the observation that the high density , small , resting B-cells had negligible background proliferation and immunoglobulin secretion , while the low density , larger , activated B-cells had marked background proliferative and antibody responses .
	manualset3
250886	11	425623	7	NULL	NULL	0	NULL	antibody responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Confirmation of these results was the observation that the high density , small , resting B-cells had negligible background proliferation and immunoglobulin secretion , while the low density , larger , activated B-cells had marked background proliferative and antibody responses .
	manualset3
250887	1	425624	7	NULL	NULL	0	NULL	cell monolayers	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Confluent cell monolayers in tissue culture are fragile and can easily be mechanically disrupted , often leaving an area devoid of cells .
	manualset3
250888	2	425624	7	NULL	NULL	0	NULL	tissue culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Confluent cell monolayers in tissue culture are fragile and can easily be mechanically disrupted , often leaving an area devoid of cells .
	manualset3
250889	3	425624	7	NULL	NULL	NULL	NULL	area	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Confluent cell monolayers in tissue culture are fragile and can easily be mechanically disrupted , often leaving an area devoid of cells .
	manualset3
250890	4	425624	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Confluent cell monolayers in tissue culture are fragile and can easily be mechanically disrupted , often leaving an area devoid of cells .
	manualset3
250891	1	425625	7	NULL	NULL	0	NULL	Confocal analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Confocal analysis showed that laminin triggers distinct Ca ( 2 + ) raises , and that sperm exposed and kept in the presence of laminin fully retained their ability to rise intracellular Ca ( 2 + ) in response to zona pellucida proteins .
	manualset3
250892	2	425625	7	NULL	NULL	0	NULL	laminin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Confocal analysis showed that laminin triggers distinct Ca ( 2 + ) raises , and that sperm exposed and kept in the presence of laminin fully retained their ability to rise intracellular Ca ( 2 + ) in response to zona pellucida proteins .
	manualset3
250893	3	425625	7	NULL	NULL	0	NULL	 Ca ( 2 + )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Confocal analysis showed that laminin triggers distinct Ca ( 2 + ) raises , and that sperm exposed and kept in the presence of laminin fully retained their ability to rise intracellular Ca ( 2 + ) in response to zona pellucida proteins .
	manualset3
250894	4	425625	7	NULL	NULL	0	NULL	sperm	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Confocal analysis showed that laminin triggers distinct Ca ( 2 + ) raises , and that sperm exposed and kept in the presence of laminin fully retained their ability to rise intracellular Ca ( 2 + ) in response to zona pellucida proteins .
	manualset3
250895	5	425625	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Confocal analysis showed that laminin triggers distinct Ca ( 2 + ) raises , and that sperm exposed and kept in the presence of laminin fully retained their ability to rise intracellular Ca ( 2 + ) in response to zona pellucida proteins .
	manualset3
250897	6	425625	7	NULL	NULL	0	NULL	laminin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Confocal analysis showed that laminin triggers distinct Ca ( 2 + ) raises , and that sperm exposed and kept in the presence of laminin fully retained their ability to rise intracellular Ca ( 2 + ) in response to zona pellucida proteins .
	manualset3
250898	7	425625	7	NULL	NULL	0	NULL	ability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Confocal analysis showed that laminin triggers distinct Ca ( 2 + ) raises , and that sperm exposed and kept in the presence of laminin fully retained their ability to rise intracellular Ca ( 2 + ) in response to zona pellucida proteins .
	manualset3
250899	8	425625	7	NULL	NULL	0	NULL	 intracellular Ca ( 2 + )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Confocal analysis showed that laminin triggers distinct Ca ( 2 + ) raises , and that sperm exposed and kept in the presence of laminin fully retained their ability to rise intracellular Ca ( 2 + ) in response to zona pellucida proteins .
	manualset3
250900	9	425625	7	NULL	NULL	0	NULL	 zona pellucida proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Confocal analysis showed that laminin triggers distinct Ca ( 2 + ) raises , and that sperm exposed and kept in the presence of laminin fully retained their ability to rise intracellular Ca ( 2 + ) in response to zona pellucida proteins .
	manualset3
250901	1	425626	7	NULL	NULL	0	NULL	Confocal microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Confocal microscopy showed that PTTG-overexpressing cells have enlarged nuclei and marked redistribution of chromatin , and electron microscopy of alphaGSU .
	manualset3
250902	2	425626	7	NULL	NULL	0	NULL	PTTG-overexpressing cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Confocal microscopy showed that PTTG-overexpressing cells have enlarged nuclei and marked redistribution of chromatin , and electron microscopy of alphaGSU .
	manualset3
250903	3	425626	7	NULL	NULL	0	NULL	enlarged nuclei	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Confocal microscopy showed that PTTG-overexpressing cells have enlarged nuclei and marked redistribution of chromatin , and electron microscopy of alphaGSU .
	manualset3
250904	4	425626	7	NULL	NULL	0	NULL	marked redistribution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Confocal microscopy showed that PTTG-overexpressing cells have enlarged nuclei and marked redistribution of chromatin , and electron microscopy of alphaGSU .
	manualset3
250905	5	425626	7	NULL	NULL	0	NULL	chromatin	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Confocal microscopy showed that PTTG-overexpressing cells have enlarged nuclei and marked redistribution of chromatin , and electron microscopy of alphaGSU .
	manualset3
250906	6	425626	7	NULL	NULL	0	NULL	electron microscopy	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Confocal microscopy showed that PTTG-overexpressing cells have enlarged nuclei and marked redistribution of chromatin , and electron microscopy of alphaGSU .
	manualset3
250907	7	425626	7	NULL	NULL	0	NULL	alphaGSU	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Confocal microscopy showed that PTTG-overexpressing cells have enlarged nuclei and marked redistribution of chromatin , and electron microscopy of alphaGSU .
	manualset3
250908	1	425627	7	NULL	NULL	0	NULL	Conformation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conformation of the HIV-1 gp 120 envelope glycoprotein .
	manualset3
250909	2	425627	7	NULL	NULL	0	NULL	HIV-1 gp 120 envelope glycoprotein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Conformation of the HIV-1 gp 120 envelope glycoprotein .
	manualset3
250910	1	425628	7	NULL	NULL	0	NULL	Conformational control 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conformational control of cofactors in nature -- functional tetrapyrrole conformations in the photosynthetic reaction centers of purple bacteria .
	manualset3
250911	2	425628	7	NULL	NULL	0	NULL	cofactors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Conformational control of cofactors in nature -- functional tetrapyrrole conformations in the photosynthetic reaction centers of purple bacteria .
	manualset3
250912	3	425628	7	NULL	NULL	0	NULL	nature	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Conformational control of cofactors in nature -- functional tetrapyrrole conformations in the photosynthetic reaction centers of purple bacteria .
	manualset3
250913	4	425628	7	NULL	NULL	0	NULL	 functional tetrapyrrole conformations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Conformational control of cofactors in nature -- functional tetrapyrrole conformations in the photosynthetic reaction centers of purple bacteria .
	manualset3
250914	5	425628	7	NULL	NULL	0	NULL	 photosynthetic reaction centers	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Conformational control of cofactors in nature -- functional tetrapyrrole conformations in the photosynthetic reaction centers of purple bacteria .
	manualset3
250915	6	425628	7	NULL	NULL	0	NULL	purple bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Conformational control of cofactors in nature -- functional tetrapyrrole conformations in the photosynthetic reaction centers of purple bacteria .
	manualset3
250916	1	425629	7	NULL	NULL	0	NULL	Lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Lesions of the liver in atherosclerosis ) .
	manualset3
250917	2	425629	7	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Lesions of the liver in atherosclerosis ) .
	manualset3
250918	3	425629	7	NULL	NULL	0	NULL	atherosclerosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Lesions of the liver in atherosclerosis ) .
	manualset3
250919	1	425630	7	NULL	NULL	0	NULL	Conforming 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conforming to the RNA gel-blot analysis , DWF4 : beta-glucuronidase ( GUS ) histochemical analyses more precisely define the tissues that express the DWF4 gene .
	manualset3
250920	2	425630	7	NULL	NULL	0	NULL	RNA gel-blot analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Conforming to the RNA gel-blot analysis , DWF4 : beta-glucuronidase ( GUS ) histochemical analyses more precisely define the tissues that express the DWF4 gene .
	manualset3
250921	3	425630	7	NULL	NULL	0	NULL	DWF4 : beta-glucuronidase ( GUS ) histochemical analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Conforming to the RNA gel-blot analysis , DWF4 : beta-glucuronidase ( GUS ) histochemical analyses more precisely define the tissues that express the DWF4 gene .
	manualset3
250922	4	425630	7	NULL	NULL	0	NULL	 tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Conforming to the RNA gel-blot analysis , DWF4 : beta-glucuronidase ( GUS ) histochemical analyses more precisely define the tissues that express the DWF4 gene .
	manualset3
250923	5	425630	7	NULL	NULL	0	NULL	DWF4 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Conforming to the RNA gel-blot analysis , DWF4 : beta-glucuronidase ( GUS ) histochemical analyses more precisely define the tissues that express the DWF4 gene .
	manualset3
251149	1	425631	7	NULL	NULL	0	NULL	Congenital central hypoventilation syndrome 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Congenital central hypoventilation syndrome : a novel mutation of the RET gene in an isolated case .
	manualset3
251150	2	425631	7	NULL	NULL	0	NULL	novel mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Congenital central hypoventilation syndrome : a novel mutation of the RET gene in an isolated case .
	manualset3
251151	3	425631	7	NULL	NULL	0	NULL	RET gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Congenital central hypoventilation syndrome : a novel mutation of the RET gene in an isolated case .
	manualset3
251152	4	425631	7	NULL	NULL	0	NULL	isolated case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Congenital central hypoventilation syndrome : a novel mutation of the RET gene in an isolated case .
	manualset3
251153	1	425632	7	NULL	NULL	0	NULL	Congenital high airway obstruction syndrome 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Congenital high airway obstruction syndrome : MR/US findings , effect on management , and outcome .
	manualset3
251154	2	425632	7	NULL	NULL	0	NULL	MR/US findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Congenital high airway obstruction syndrome : MR/US findings , effect on management , and outcome .
	manualset3
251155	3	425632	7	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Congenital high airway obstruction syndrome : MR/US findings , effect on management , and outcome .
	manualset3
251156	4	425632	7	NULL	NULL	0	NULL	management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Congenital high airway obstruction syndrome : MR/US findings , effect on management , and outcome .
	manualset3
251157	5	425632	7	NULL	NULL	0	NULL	outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Congenital high airway obstruction syndrome : MR/US findings , effect on management , and outcome .
	manualset3
251158	1	425633	7	NULL	NULL	0	NULL	recipient 's bodily expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Congruence between the recipient 's bodily expression of emotion and the sender 's emotional tone of language , for instance , facilitates comprehension of the communication , whereas incongruence can impair comprehension .
	manualset3
251159	2	425633	7	NULL	NULL	0	NULL	emotion	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Congruence between the recipient 's bodily expression of emotion and the sender 's emotional tone of language , for instance , facilitates comprehension of the communication , whereas incongruence can impair comprehension .
	manualset3
251161	3	425633	7	NULL	NULL	0	NULL	sender 's emotional tone of language	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Congruence between the recipient 's bodily expression of emotion and the sender 's emotional tone of language , for instance , facilitates comprehension of the communication , whereas incongruence can impair comprehension .
	manualset3
251162	4	425633	7	NULL	NULL	0	NULL	comprehension	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Congruence between the recipient 's bodily expression of emotion and the sender 's emotional tone of language , for instance , facilitates comprehension of the communication , whereas incongruence can impair comprehension .
	manualset3
251163	5	425633	7	NULL	NULL	0	NULL	communication	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Congruence between the recipient 's bodily expression of emotion and the sender 's emotional tone of language , for instance , facilitates comprehension of the communication , whereas incongruence can impair comprehension .
	manualset3
251164	6	425633	7	NULL	NULL	0	NULL	comprehension	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Congruence between the recipient 's bodily expression of emotion and the sender 's emotional tone of language , for instance , facilitates comprehension of the communication , whereas incongruence can impair comprehension .
	manualset3
251170	1	425634	7	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Congruously , cells derived from OS patients that carry MID1 mutations exhibit decreased mTORC1 formation , S6K1 phosphorylation , cell size , and cap-dependent translation , all of which is rescued by expression of wild-type MID1 or an activated mTOR allele .
	manualset3
251171	2	425634	7	NULL	NULL	0	NULL	OS patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Congruously , cells derived from OS patients that carry MID1 mutations exhibit decreased mTORC1 formation , S6K1 phosphorylation , cell size , and cap-dependent translation , all of which is rescued by expression of wild-type MID1 or an activated mTOR allele .
	manualset3
251172	3	425634	7	NULL	NULL	0	NULL	MID1 mutations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Congruously , cells derived from OS patients that carry MID1 mutations exhibit decreased mTORC1 formation , S6K1 phosphorylation , cell size , and cap-dependent translation , all of which is rescued by expression of wild-type MID1 or an activated mTOR allele .
	manualset3
251174	4	425634	7	NULL	NULL	0	NULL	mTORC1 formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Congruously , cells derived from OS patients that carry MID1 mutations exhibit decreased mTORC1 formation , S6K1 phosphorylation , cell size , and cap-dependent translation , all of which is rescued by expression of wild-type MID1 or an activated mTOR allele .
	manualset3
251176	5	425634	7	NULL	NULL	0	NULL	S6K1 phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Congruously , cells derived from OS patients that carry MID1 mutations exhibit decreased mTORC1 formation , S6K1 phosphorylation , cell size , and cap-dependent translation , all of which is rescued by expression of wild-type MID1 or an activated mTOR allele .
	manualset3
251177	6	425634	7	NULL	NULL	0	NULL	cell size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Congruously , cells derived from OS patients that carry MID1 mutations exhibit decreased mTORC1 formation , S6K1 phosphorylation , cell size , and cap-dependent translation , all of which is rescued by expression of wild-type MID1 or an activated mTOR allele .
	manualset3
251179	7	425634	7	NULL	NULL	0	NULL	cap-dependent translation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Congruously , cells derived from OS patients that carry MID1 mutations exhibit decreased mTORC1 formation , S6K1 phosphorylation , cell size , and cap-dependent translation , all of which is rescued by expression of wild-type MID1 or an activated mTOR allele .
	manualset3
251181	8	425634	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Congruously , cells derived from OS patients that carry MID1 mutations exhibit decreased mTORC1 formation , S6K1 phosphorylation , cell size , and cap-dependent translation , all of which is rescued by expression of wild-type MID1 or an activated mTOR allele .
	manualset3
251182	9	425634	7	NULL	NULL	0	NULL	wild-type MID1 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Congruously , cells derived from OS patients that carry MID1 mutations exhibit decreased mTORC1 formation , S6K1 phosphorylation , cell size , and cap-dependent translation , all of which is rescued by expression of wild-type MID1 or an activated mTOR allele .
	manualset3
251183	10	425634	7	NULL	NULL	0	NULL	activated mTOR allele	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Congruously , cells derived from OS patients that carry MID1 mutations exhibit decreased mTORC1 formation , S6K1 phosphorylation , cell size , and cap-dependent translation , all of which is rescued by expression of wild-type MID1 or an activated mTOR allele .
	manualset3
251184	1	425635	7	NULL	NULL	0	NULL	Conifer needles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Conifer needles as passive biomonitors of the spatial and temporal distribution of DDT from a point source .
	manualset3
251187	2	425635	7	NULL	NULL	0	NULL	passive biomonitors 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Conifer needles as passive biomonitors of the spatial and temporal distribution of DDT from a point source .
	manualset3
251190	3	425635	7	NULL	NULL	0	NULL	spatial distribution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Conifer needles as passive biomonitors of the spatial and temporal distribution of DDT from a point source .
	manualset3
251191	4	425635	7	NULL	NULL	0	NULL	 temporal distribution 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Conifer needles as passive biomonitors of the spatial and temporal distribution of DDT from a point source .
	manualset3
251192	5	425635	7	NULL	NULL	0	NULL	DDT 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Conifer needles as passive biomonitors of the spatial and temporal distribution of DDT from a point source .
	manualset3
251193	6	425635	7	NULL	NULL	0	NULL	point source	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Conifer needles as passive biomonitors of the spatial and temporal distribution of DDT from a point source .
	manualset3
251194	1	425636	7	NULL	NULL	0	NULL	Conjunctival thickness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conjunctival thickness served as a reliable indicator of anaphylaxis .
	manualset3
251195	2	425636	7	NULL	NULL	0	NULL	reliable indicator 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conjunctival thickness served as a reliable indicator of anaphylaxis .
	manualset3
251196	3	425636	7	NULL	NULL	0	NULL	anaphylaxis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conjunctival thickness served as a reliable indicator of anaphylaxis .
	manualset3
251197	1	425637	7	NULL	NULL	0	NULL	 Letter	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Letter : Acute lymphoid leukemia : constant induction of remission by the combination of prednisone , vincristine and L-asparaginase ( 20 cases ) ) .
	manualset3
251198	2	425637	7	NULL	NULL	0	NULL	Acute lymphoid leukemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Letter : Acute lymphoid leukemia : constant induction of remission by the combination of prednisone , vincristine and L-asparaginase ( 20 cases ) ) .
	manualset3
251199	3	425637	7	NULL	NULL	0	NULL	constant induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Letter : Acute lymphoid leukemia : constant induction of remission by the combination of prednisone , vincristine and L-asparaginase ( 20 cases ) ) .
	manualset3
251200	4	425637	7	NULL	NULL	0	NULL	remission	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Letter : Acute lymphoid leukemia : constant induction of remission by the combination of prednisone , vincristine and L-asparaginase ( 20 cases ) ) .
	manualset3
251201	5	425637	7	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Letter : Acute lymphoid leukemia : constant induction of remission by the combination of prednisone , vincristine and L-asparaginase ( 20 cases ) ) .
	manualset3
251202	6	425637	7	NULL	NULL	NULL	NULL	prednisone	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Letter : Acute lymphoid leukemia : constant induction of remission by the combination of prednisone , vincristine and L-asparaginase ( 20 cases ) ) .
	manualset3
251203	7	425637	7	NULL	NULL	0	NULL	vincristine 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Letter : Acute lymphoid leukemia : constant induction of remission by the combination of prednisone , vincristine and L-asparaginase ( 20 cases ) ) .
	manualset3
251204	8	425637	7	NULL	NULL	0	NULL	L-asparaginase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Letter : Acute lymphoid leukemia : constant induction of remission by the combination of prednisone , vincristine and L-asparaginase ( 20 cases ) ) .
	manualset3
251205	9	425637	7	NULL	NULL	0	NULL	20 cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Letter : Acute lymphoid leukemia : constant induction of remission by the combination of prednisone , vincristine and L-asparaginase ( 20 cases ) ) .
	manualset3
251216	1	425638	7	NULL	NULL	0	NULL	Conmen 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Conmen and confusion : consumer fraud and vulnerable older people in the community .
	manualset3
251217	2	425638	7	NULL	NULL	0	NULL	confusion	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Conmen and confusion : consumer fraud and vulnerable older people in the community .
	manualset3
251218	3	425638	7	NULL	NULL	0	NULL	 consumer fraud	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conmen and confusion : consumer fraud and vulnerable older people in the community .
	manualset3
251219	4	425638	7	NULL	NULL	0	NULL	older people 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Conmen and confusion : consumer fraud and vulnerable older people in the community .
	manualset3
251220	5	425638	7	NULL	NULL	0	NULL	community	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Conmen and confusion : consumer fraud and vulnerable older people in the community .
	manualset3
251221	1	425639	7	NULL	NULL	0	NULL	Connections	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Connections also exist with conductive media such as cerebrospinal fluid , bile , and urine .
	manualset3
251222	2	425639	7	NULL	NULL	0	NULL	conductive media	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Connections also exist with conductive media such as cerebrospinal fluid , bile , and urine .
	manualset3
251223	3	425639	7	NULL	NULL	0	NULL	cerebrospinal fluid 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Connections also exist with conductive media such as cerebrospinal fluid , bile , and urine .
	manualset3
251224	4	425639	7	NULL	NULL	0	NULL	bile	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Connections also exist with conductive media such as cerebrospinal fluid , bile , and urine .
	manualset3
251225	5	425639	7	NULL	NULL	0	NULL	urine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Connections also exist with conductive media such as cerebrospinal fluid , bile , and urine .
	manualset3
251226	1	425640	7	NULL	NULL	0	NULL	Connexin channels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Connexin channels mediate electrical synaptic transmission when assembled as cell-to-cell pores at gap junctions and can mediate transmembrane currents when expressed in plasma membranes as hemichannels .
	manualset3
251227	2	425640	7	NULL	NULL	0	NULL	electrical synaptic transmission	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Connexin channels mediate electrical synaptic transmission when assembled as cell-to-cell pores at gap junctions and can mediate transmembrane currents when expressed in plasma membranes as hemichannels .
	manualset3
251228	3	425640	7	NULL	NULL	0	NULL	 cell-to-cell pores	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Connexin channels mediate electrical synaptic transmission when assembled as cell-to-cell pores at gap junctions and can mediate transmembrane currents when expressed in plasma membranes as hemichannels .
	manualset3
251229	4	425640	7	NULL	NULL	0	NULL	gap junctions	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Connexin channels mediate electrical synaptic transmission when assembled as cell-to-cell pores at gap junctions and can mediate transmembrane currents when expressed in plasma membranes as hemichannels .
	manualset3
251230	5	425640	7	NULL	NULL	0	NULL	transmembrane currents	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Connexin channels mediate electrical synaptic transmission when assembled as cell-to-cell pores at gap junctions and can mediate transmembrane currents when expressed in plasma membranes as hemichannels .
	manualset3
251231	6	425640	7	NULL	NULL	0	NULL	plasma membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Connexin channels mediate electrical synaptic transmission when assembled as cell-to-cell pores at gap junctions and can mediate transmembrane currents when expressed in plasma membranes as hemichannels .
	manualset3
251232	7	425640	7	NULL	NULL	0	NULL	hemichannels	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Connexin channels mediate electrical synaptic transmission when assembled as cell-to-cell pores at gap junctions and can mediate transmembrane currents when expressed in plasma membranes as hemichannels .
	manualset3
251233	1	425641	7	NULL	NULL	0	NULL	 tuberculosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Conquering tuberculosis : dream or reality ?
	manualset3
251234	2	425641	7	NULL	NULL	0	NULL	dream	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Conquering tuberculosis : dream or reality ?
	manualset3
251235	3	425641	7	NULL	NULL	0	NULL	reality	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conquering tuberculosis : dream or reality ?
	manualset3
251236	1	425642	7	NULL	NULL	0	NULL	 concomitant administration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , concomitant administration of small molecule inhibitors of the VEGF pathway will likely have a positive impact on chemoradiation treatment outcome .
	manualset3
251237	2	425642	7	NULL	NULL	0	NULL	small molecule inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , concomitant administration of small molecule inhibitors of the VEGF pathway will likely have a positive impact on chemoradiation treatment outcome .
	manualset3
251239	3	425642	7	NULL	NULL	0	NULL	VEGF pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , concomitant administration of small molecule inhibitors of the VEGF pathway will likely have a positive impact on chemoradiation treatment outcome .
	manualset3
251240	4	425642	7	NULL	NULL	0	NULL	 positive impact 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , concomitant administration of small molecule inhibitors of the VEGF pathway will likely have a positive impact on chemoradiation treatment outcome .
	manualset3
251242	5	425642	7	NULL	NULL	0	NULL	chemoradiation treatment outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , concomitant administration of small molecule inhibitors of the VEGF pathway will likely have a positive impact on chemoradiation treatment outcome .
	manualset3
251245	1	425643	7	NULL	NULL	0	NULL	 summer	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , during summer under the influence of changing day-length the thermal requirements for development in many insects gradually vary , which may have adaptive significance .
	manualset3
251246	2	425643	7	NULL	NULL	0	NULL	influence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , during summer under the influence of changing day-length the thermal requirements for development in many insects gradually vary , which may have adaptive significance .
	manualset3
251247	3	425643	7	NULL	NULL	NULL	NULL	changing day-length	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Consequently , during summer under the influence of changing day-length the thermal requirements for development in many insects gradually vary , which may have adaptive significance .
	manualset3
251248	4	425643	7	NULL	NULL	NULL	NULL	thermal requirements	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Consequently , during summer under the influence of changing day-length the thermal requirements for development in many insects gradually vary , which may have adaptive significance .
	manualset3
251258	5	425643	7	NULL	NULL	0	NULL	 development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , during summer under the influence of changing day-length the thermal requirements for development in many insects gradually vary , which may have adaptive significance .
	manualset3
251260	6	425643	7	NULL	NULL	0	NULL	 insects	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , during summer under the influence of changing day-length the thermal requirements for development in many insects gradually vary , which may have adaptive significance .
	manualset3
254090	7	425643	7	NULL	NULL	NULL	NULL	adaptive significance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Consequently , during summer under the influence of changing day-length the thermal requirements for development in many insects gradually vary , which may have adaptive significance .
	manualset3
251261	1	425644	7	NULL	NULL	0	NULL	Leukemia morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Leukemia morbidity in Samarkand and the Samarkand region from 1966 to 1969 ) .
	manualset3
251262	2	425644	7	NULL	NULL	0	NULL	 Samarkand	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Leukemia morbidity in Samarkand and the Samarkand region from 1966 to 1969 ) .
	manualset3
251267	3	425644	7	NULL	NULL	0	NULL	Samarkand region	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Leukemia morbidity in Samarkand and the Samarkand region from 1966 to 1969 ) .
	manualset3
251269	4	425644	7	NULL	NULL	0	NULL	1966	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	( Leukemia morbidity in Samarkand and the Samarkand region from 1966 to 1969 ) .
	manualset3
251271	5	425644	7	NULL	NULL	0	NULL	1969	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	( Leukemia morbidity in Samarkand and the Samarkand region from 1966 to 1969 ) .
	manualset3
251275	1	425645	7	NULL	NULL	0	NULL	immunomodulation 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , immunomodulation by dietary polyunsaturated fatty acids may have profound effects at secondary rather than at primary exposure to pathogens .
	manualset3
251276	2	425645	7	NULL	NULL	0	NULL	dietary polyunsaturated fatty acids	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , immunomodulation by dietary polyunsaturated fatty acids may have profound effects at secondary rather than at primary exposure to pathogens .
	manualset3
251277	3	425645	7	NULL	NULL	0	NULL	profound effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , immunomodulation by dietary polyunsaturated fatty acids may have profound effects at secondary rather than at primary exposure to pathogens .
	manualset3
251278	4	425645	7	NULL	NULL	0	NULL	primary exposure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , immunomodulation by dietary polyunsaturated fatty acids may have profound effects at secondary rather than at primary exposure to pathogens .
	manualset3
251279	5	425645	7	NULL	NULL	0	NULL	pathogens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , immunomodulation by dietary polyunsaturated fatty acids may have profound effects at secondary rather than at primary exposure to pathogens .
	manualset3
251280	1	425646	7	NULL	NULL	0	NULL	inadvertent placement 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , inadvertent placement of the needle into the vertebral artery , thyroid , neural tissues , or esophagus can occur with the fluoroscopic or blind approach .
	manualset3
251281	2	425646	7	NULL	NULL	0	NULL	 needle	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , inadvertent placement of the needle into the vertebral artery , thyroid , neural tissues , or esophagus can occur with the fluoroscopic or blind approach .
	manualset3
251282	3	425646	7	NULL	NULL	0	NULL	vertebral artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , inadvertent placement of the needle into the vertebral artery , thyroid , neural tissues , or esophagus can occur with the fluoroscopic or blind approach .
	manualset3
251283	4	425646	7	NULL	NULL	0	NULL	thyroid	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , inadvertent placement of the needle into the vertebral artery , thyroid , neural tissues , or esophagus can occur with the fluoroscopic or blind approach .
	manualset3
251285	5	425646	7	NULL	NULL	0	NULL	esophagus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , inadvertent placement of the needle into the vertebral artery , thyroid , neural tissues , or esophagus can occur with the fluoroscopic or blind approach .
	manualset3
251287	6	425646	7	NULL	NULL	0	NULL	 fluoroscopic approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , inadvertent placement of the needle into the vertebral artery , thyroid , neural tissues , or esophagus can occur with the fluoroscopic or blind approach .
	manualset3
251289	7	425646	7	NULL	NULL	0	NULL	blind approach	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , inadvertent placement of the needle into the vertebral artery , thyroid , neural tissues , or esophagus can occur with the fluoroscopic or blind approach .
	manualset3
254091	8	425646	7	NULL	NULL	NULL	NULL	neural tissues	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Consequently , inadvertent placement of the needle into the vertebral artery , thyroid , neural tissues , or esophagus can occur with the fluoroscopic or blind approach .
	manualset3
251293	1	425647	7	NULL	NULL	0	NULL	 inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , inhibition of ALDH2 would lead to elevated levels of acetaldehyde and other reactive lipid peroxides following ethanol intake and/or exposure to toxic chemicals .
	manualset3
251295	2	425647	7	NULL	NULL	0	NULL	ALDH2 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , inhibition of ALDH2 would lead to elevated levels of acetaldehyde and other reactive lipid peroxides following ethanol intake and/or exposure to toxic chemicals .
	manualset3
251297	3	425647	7	NULL	NULL	0	NULL	 elevated levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , inhibition of ALDH2 would lead to elevated levels of acetaldehyde and other reactive lipid peroxides following ethanol intake and/or exposure to toxic chemicals .
	manualset3
251299	4	425647	7	NULL	NULL	0	NULL	 acetaldehyde	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , inhibition of ALDH2 would lead to elevated levels of acetaldehyde and other reactive lipid peroxides following ethanol intake and/or exposure to toxic chemicals .
	manualset3
251300	5	425647	7	NULL	NULL	NULL	NULL	reactive lipid peroxides	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Consequently , inhibition of ALDH2 would lead to elevated levels of acetaldehyde and other reactive lipid peroxides following ethanol intake and/or exposure to toxic chemicals .
	manualset3
251301	6	425647	7	NULL	NULL	0	NULL	ethanol intake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , inhibition of ALDH2 would lead to elevated levels of acetaldehyde and other reactive lipid peroxides following ethanol intake and/or exposure to toxic chemicals .
	manualset3
251302	7	425647	7	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , inhibition of ALDH2 would lead to elevated levels of acetaldehyde and other reactive lipid peroxides following ethanol intake and/or exposure to toxic chemicals .
	manualset3
251303	8	425647	7	NULL	NULL	0	NULL	toxic chemicals	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , inhibition of ALDH2 would lead to elevated levels of acetaldehyde and other reactive lipid peroxides following ethanol intake and/or exposure to toxic chemicals .
	manualset3
251306	1	425648	7	NULL	NULL	0	NULL	F forms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , the F forms show prolonged and more reproducible GRTs compared to the NF ones .
	manualset3
251311	2	425648	7	NULL	NULL	0	NULL	reproducible GRTs	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , the F forms show prolonged and more reproducible GRTs compared to the NF ones .
	manualset3
251312	3	425648	7	NULL	NULL	0	NULL	NF ones	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , the F forms show prolonged and more reproducible GRTs compared to the NF ones .
	manualset3
251329	1	425649	7	NULL	NULL	0	NULL	 lack	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , the lack of aflatoxin-producing ability of A. sojae resulted primarily from two defects in the regulatory mechanism responsible for gene transcription .
	manualset3
251331	2	425649	7	NULL	NULL	0	NULL	aflatoxin-producing ability 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , the lack of aflatoxin-producing ability of A. sojae resulted primarily from two defects in the regulatory mechanism responsible for gene transcription .
	manualset3
251332	3	425649	7	NULL	NULL	0	NULL	A. sojae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , the lack of aflatoxin-producing ability of A. sojae resulted primarily from two defects in the regulatory mechanism responsible for gene transcription .
	manualset3
251339	4	425649	7	NULL	NULL	NULL	NULL	two defects 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Consequently , the lack of aflatoxin-producing ability of A. sojae resulted primarily from two defects in the regulatory mechanism responsible for gene transcription .
	manualset3
251342	5	425649	7	NULL	NULL	0	NULL	 regulatory mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , the lack of aflatoxin-producing ability of A. sojae resulted primarily from two defects in the regulatory mechanism responsible for gene transcription .
	manualset3
251343	6	425649	7	NULL	NULL	0	NULL	 gene transcription	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , the lack of aflatoxin-producing ability of A. sojae resulted primarily from two defects in the regulatory mechanism responsible for gene transcription .
	manualset3
251345	1	425650	7	NULL	NULL	0	NULL	current information	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , we have chosen to summarize the current information on a subset of TGF ligand and receptor genes and related effector genes that , when dysregulated , are known to lead to cardiovascular diseases and adult cardiovascular deficiencies and/or pathologies .
	manualset3
251348	2	425650	7	NULL	NULL	0	NULL	 subset	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , we have chosen to summarize the current information on a subset of TGF ligand and receptor genes and related effector genes that , when dysregulated , are known to lead to cardiovascular diseases and adult cardiovascular deficiencies and/or pathologies .
	manualset3
251350	3	425650	7	NULL	NULL	0	NULL	TGF ligand 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , we have chosen to summarize the current information on a subset of TGF ligand and receptor genes and related effector genes that , when dysregulated , are known to lead to cardiovascular diseases and adult cardiovascular deficiencies and/or pathologies .
	manualset3
251353	4	425650	7	NULL	NULL	0	NULL	receptor genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , we have chosen to summarize the current information on a subset of TGF ligand and receptor genes and related effector genes that , when dysregulated , are known to lead to cardiovascular diseases and adult cardiovascular deficiencies and/or pathologies .
	manualset3
251354	5	425650	7	NULL	NULL	0	NULL	related effector genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , we have chosen to summarize the current information on a subset of TGF ligand and receptor genes and related effector genes that , when dysregulated , are known to lead to cardiovascular diseases and adult cardiovascular deficiencies and/or pathologies .
	manualset3
251356	6	425650	7	NULL	NULL	0	NULL	cardiovascular diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , we have chosen to summarize the current information on a subset of TGF ligand and receptor genes and related effector genes that , when dysregulated , are known to lead to cardiovascular diseases and adult cardiovascular deficiencies and/or pathologies .
	manualset3
251357	7	425650	7	NULL	NULL	0	NULL	adult cardiovascular deficiencies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , we have chosen to summarize the current information on a subset of TGF ligand and receptor genes and related effector genes that , when dysregulated , are known to lead to cardiovascular diseases and adult cardiovascular deficiencies and/or pathologies .
	manualset3
251358	8	425650	7	NULL	NULL	0	NULL	pathologies	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently , we have chosen to summarize the current information on a subset of TGF ligand and receptor genes and related effector genes that , when dysregulated , are known to lead to cardiovascular diseases and adult cardiovascular deficiencies and/or pathologies .
	manualset3
251366	1	425651	7	NULL	NULL	0	NULL	LRP1B expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently LRP1B expression could function to protect against the pathogenesis of Alzheimer 's disease .
	manualset3
251367	2	425651	7	NULL	NULL	0	NULL	 pathogenesis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently LRP1B expression could function to protect against the pathogenesis of Alzheimer 's disease .
	manualset3
251368	3	425651	7	NULL	NULL	0	NULL	Alzheimer 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Consequently LRP1B expression could function to protect against the pathogenesis of Alzheimer 's disease .
	manualset3
251371	1	425652	7	NULL	NULL	0	NULL	 Leukocyte depletion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Leukocyte depletion by in-line-filtration ) .
	manualset3
251373	2	425652	7	NULL	NULL	0	NULL	in-line-filtration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Leukocyte depletion by in-line-filtration ) .
	manualset3
251376	1	425653	7	NULL	NULL	0	NULL	Conservation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conservation of the linkage relationships of markers in the FAD region suggests that the murine homolog of the FAD locus probably maps to chromosome 16 and that detailed comparison of the corresponding region in both species could facilitate identification of the primary defect in this disorder .
	manualset3
251377	2	425653	7	NULL	NULL	0	NULL	linkage relationships	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Conservation of the linkage relationships of markers in the FAD region suggests that the murine homolog of the FAD locus probably maps to chromosome 16 and that detailed comparison of the corresponding region in both species could facilitate identification of the primary defect in this disorder .
	manualset3
251378	3	425653	7	NULL	NULL	0	NULL	markers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Conservation of the linkage relationships of markers in the FAD region suggests that the murine homolog of the FAD locus probably maps to chromosome 16 and that detailed comparison of the corresponding region in both species could facilitate identification of the primary defect in this disorder .
	manualset3
251379	4	425653	7	NULL	NULL	0	NULL	FAD region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Conservation of the linkage relationships of markers in the FAD region suggests that the murine homolog of the FAD locus probably maps to chromosome 16 and that detailed comparison of the corresponding region in both species could facilitate identification of the primary defect in this disorder .
	manualset3
251380	5	425653	7	NULL	NULL	0	NULL	murine homolog	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Conservation of the linkage relationships of markers in the FAD region suggests that the murine homolog of the FAD locus probably maps to chromosome 16 and that detailed comparison of the corresponding region in both species could facilitate identification of the primary defect in this disorder .
	manualset3
251381	6	425653	7	NULL	NULL	0	NULL	FAD locus	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Conservation of the linkage relationships of markers in the FAD region suggests that the murine homolog of the FAD locus probably maps to chromosome 16 and that detailed comparison of the corresponding region in both species could facilitate identification of the primary defect in this disorder .
	manualset3
251382	7	425653	7	NULL	NULL	0	NULL	chromosome 16 	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Conservation of the linkage relationships of markers in the FAD region suggests that the murine homolog of the FAD locus probably maps to chromosome 16 and that detailed comparison of the corresponding region in both species could facilitate identification of the primary defect in this disorder .
	manualset3
251383	8	425653	7	NULL	NULL	0	NULL	 comparison	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conservation of the linkage relationships of markers in the FAD region suggests that the murine homolog of the FAD locus probably maps to chromosome 16 and that detailed comparison of the corresponding region in both species could facilitate identification of the primary defect in this disorder .
	manualset3
251384	9	425653	7	NULL	NULL	0	NULL	corresponding region 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Conservation of the linkage relationships of markers in the FAD region suggests that the murine homolog of the FAD locus probably maps to chromosome 16 and that detailed comparison of the corresponding region in both species could facilitate identification of the primary defect in this disorder .
	manualset3
251385	10	425653	7	NULL	NULL	0	NULL	species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Conservation of the linkage relationships of markers in the FAD region suggests that the murine homolog of the FAD locus probably maps to chromosome 16 and that detailed comparison of the corresponding region in both species could facilitate identification of the primary defect in this disorder .
	manualset3
251386	11	425653	7	NULL	NULL	0	NULL	identification 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conservation of the linkage relationships of markers in the FAD region suggests that the murine homolog of the FAD locus probably maps to chromosome 16 and that detailed comparison of the corresponding region in both species could facilitate identification of the primary defect in this disorder .
	manualset3
251387	12	425653	7	NULL	NULL	0	NULL	primary defect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conservation of the linkage relationships of markers in the FAD region suggests that the murine homolog of the FAD locus probably maps to chromosome 16 and that detailed comparison of the corresponding region in both species could facilitate identification of the primary defect in this disorder .
	manualset3
251388	13	425653	7	NULL	NULL	0	NULL	 disorder	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conservation of the linkage relationships of markers in the FAD region suggests that the murine homolog of the FAD locus probably maps to chromosome 16 and that detailed comparison of the corresponding region in both species could facilitate identification of the primary defect in this disorder .
	manualset3
251389	1	425654	7	NULL	NULL	0	NULL	Conserved charged amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Conserved charged amino acids on one side of the beta-propeller structure were found to confer most of the 40S subunit binding affinity , whereas an adjacent conserved and structured loop had little effect on RACK1-ribosome association .
	manualset3
251390	2	425654	7	NULL	NULL	0	NULL	one side	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Conserved charged amino acids on one side of the beta-propeller structure were found to confer most of the 40S subunit binding affinity , whereas an adjacent conserved and structured loop had little effect on RACK1-ribosome association .
	manualset3
251391	4	425654	7	NULL	NULL	NULL	NULL	40S subunit binding affinity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Conserved charged amino acids on one side of the beta-propeller structure were found to confer most of the 40S subunit binding affinity , whereas an adjacent conserved and structured loop had little effect on RACK1-ribosome association .
	manualset3
251392	3	425654	7	NULL	NULL	0	NULL	beta-propeller structure	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Conserved charged amino acids on one side of the beta-propeller structure were found to confer most of the 40S subunit binding affinity , whereas an adjacent conserved and structured loop had little effect on RACK1-ribosome association .
	manualset3
251393	5	425654	7	NULL	NULL	0	NULL	conserved and structured loop 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Conserved charged amino acids on one side of the beta-propeller structure were found to confer most of the 40S subunit binding affinity , whereas an adjacent conserved and structured loop had little effect on RACK1-ribosome association .
	manualset3
251394	6	425654	7	NULL	NULL	0	NULL	effect	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Conserved charged amino acids on one side of the beta-propeller structure were found to confer most of the 40S subunit binding affinity , whereas an adjacent conserved and structured loop had little effect on RACK1-ribosome association .
	manualset3
251395	7	425654	7	NULL	NULL	0	NULL	RACK1-ribosome association	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Conserved charged amino acids on one side of the beta-propeller structure were found to confer most of the 40S subunit binding affinity , whereas an adjacent conserved and structured loop had little effect on RACK1-ribosome association .
	manualset3
251399	1	425655	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Considerable evidence now documents that the most effective ( and cost-effective ) fall reduction programs have involved systematic fall risk assessment and targeted interventions , exercise programs and environmental-inspection and hazard-reduction programs .
	manualset3
251400	2	425655	7	NULL	NULL	0	NULL	fall reduction programs	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Considerable evidence now documents that the most effective ( and cost-effective ) fall reduction programs have involved systematic fall risk assessment and targeted interventions , exercise programs and environmental-inspection and hazard-reduction programs .
	manualset3
251401	3	425655	7	NULL	NULL	0	NULL	systematic fall risk assessment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Considerable evidence now documents that the most effective ( and cost-effective ) fall reduction programs have involved systematic fall risk assessment and targeted interventions , exercise programs and environmental-inspection and hazard-reduction programs .
	manualset3
251402	4	425655	7	NULL	NULL	0	NULL	targeted interventions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Considerable evidence now documents that the most effective ( and cost-effective ) fall reduction programs have involved systematic fall risk assessment and targeted interventions , exercise programs and environmental-inspection and hazard-reduction programs .
	manualset3
251406	5	425655	7	NULL	NULL	0	NULL	exercise programs	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Considerable evidence now documents that the most effective ( and cost-effective ) fall reduction programs have involved systematic fall risk assessment and targeted interventions , exercise programs and environmental-inspection and hazard-reduction programs .
	manualset3
251407	6	425655	7	NULL	NULL	0	NULL	environmental-inspection programs	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Considerable evidence now documents that the most effective ( and cost-effective ) fall reduction programs have involved systematic fall risk assessment and targeted interventions , exercise programs and environmental-inspection and hazard-reduction programs .
	manualset3
251409	7	425655	7	NULL	NULL	0	NULL	hazard-reduction programs	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Considerable evidence now documents that the most effective ( and cost-effective ) fall reduction programs have involved systematic fall risk assessment and targeted interventions , exercise programs and environmental-inspection and hazard-reduction programs .
	manualset3
251410	1	425656	7	NULL	NULL	0	NULL	latitude 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Considerable latitude exists in the application of locomotor training , and training protocols vary widely between experimenters and clinical settings .
	manualset3
251411	2	425656	7	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Considerable latitude exists in the application of locomotor training , and training protocols vary widely between experimenters and clinical settings .
	manualset3
251413	3	425656	7	NULL	NULL	0	NULL	locomotor training 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Considerable latitude exists in the application of locomotor training , and training protocols vary widely between experimenters and clinical settings .
	manualset3
251414	4	425656	7	NULL	NULL	0	NULL	training protocols	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Considerable latitude exists in the application of locomotor training , and training protocols vary widely between experimenters and clinical settings .
	manualset3
251416	5	425656	7	NULL	NULL	0	NULL	experimenters	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Considerable latitude exists in the application of locomotor training , and training protocols vary widely between experimenters and clinical settings .
	manualset3
251417	6	425656	7	NULL	NULL	0	NULL	clinical settings	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Considerable latitude exists in the application of locomotor training , and training protocols vary widely between experimenters and clinical settings .
	manualset3
251423	1	425657	7	NULL	NULL	0	NULL	procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Consideration for this procedure requires pain of at least a 1-year duration , failure of conservative management , pain localization at a Tinel 's point , and at least a 5-point reduction of pain on a visual analog scale after nerve blockade with 1 % lidocaine .
	manualset3
251424	2	425657	7	NULL	NULL	0	NULL	pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Consideration for this procedure requires pain of at least a 1-year duration , failure of conservative management , pain localization at a Tinel 's point , and at least a 5-point reduction of pain on a visual analog scale after nerve blockade with 1 % lidocaine .
	manualset3
251427	3	425657	7	NULL	NULL	0	NULL	1-year duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Consideration for this procedure requires pain of at least a 1-year duration , failure of conservative management , pain localization at a Tinel 's point , and at least a 5-point reduction of pain on a visual analog scale after nerve blockade with 1 % lidocaine .
	manualset3
251429	4	425657	7	NULL	NULL	NULL	NULL	failure	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Consideration for this procedure requires pain of at least a 1-year duration , failure of conservative management , pain localization at a Tinel 's point , and at least a 5-point reduction of pain on a visual analog scale after nerve blockade with 1 % lidocaine .
	manualset3
251432	5	425657	7	NULL	NULL	0	NULL	conservative management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Consideration for this procedure requires pain of at least a 1-year duration , failure of conservative management , pain localization at a Tinel 's point , and at least a 5-point reduction of pain on a visual analog scale after nerve blockade with 1 % lidocaine .
	manualset3
251435	6	425657	7	NULL	NULL	0	NULL	pain localization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Consideration for this procedure requires pain of at least a 1-year duration , failure of conservative management , pain localization at a Tinel 's point , and at least a 5-point reduction of pain on a visual analog scale after nerve blockade with 1 % lidocaine .
	manualset3
251437	7	425657	7	NULL	NULL	0	NULL	Tinel 's point	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Consideration for this procedure requires pain of at least a 1-year duration , failure of conservative management , pain localization at a Tinel 's point , and at least a 5-point reduction of pain on a visual analog scale after nerve blockade with 1 % lidocaine .
	manualset3
251438	8	425657	7	NULL	NULL	0	NULL	 5-point reduction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Consideration for this procedure requires pain of at least a 1-year duration , failure of conservative management , pain localization at a Tinel 's point , and at least a 5-point reduction of pain on a visual analog scale after nerve blockade with 1 % lidocaine .
	manualset3
251440	9	425657	7	NULL	NULL	0	NULL	pain 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Consideration for this procedure requires pain of at least a 1-year duration , failure of conservative management , pain localization at a Tinel 's point , and at least a 5-point reduction of pain on a visual analog scale after nerve blockade with 1 % lidocaine .
	manualset3
251442	10	425657	7	NULL	NULL	0	NULL	visual analog scale	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Consideration for this procedure requires pain of at least a 1-year duration , failure of conservative management , pain localization at a Tinel 's point , and at least a 5-point reduction of pain on a visual analog scale after nerve blockade with 1 % lidocaine .
	manualset3
251444	11	425657	7	NULL	NULL	NULL	NULL	 nerve blockade	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Consideration for this procedure requires pain of at least a 1-year duration , failure of conservative management , pain localization at a Tinel 's point , and at least a 5-point reduction of pain on a visual analog scale after nerve blockade with 1 % lidocaine .
	manualset3
251447	12	425657	7	NULL	NULL	0	NULL	 1 % lidocaine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Consideration for this procedure requires pain of at least a 1-year duration , failure of conservative management , pain localization at a Tinel 's point , and at least a 5-point reduction of pain on a visual analog scale after nerve blockade with 1 % lidocaine .
	manualset3
254092	13	425657	7	NULL	NULL	NULL	NULL	Consideration	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Consideration for this procedure requires pain of at least a 1-year duration , failure of conservative management , pain localization at a Tinel 's point , and at least a 5-point reduction of pain on a visual analog scale after nerve blockade with 1 % lidocaine .
	manualset3
251597	1	425658	7	NULL	NULL	NULL	NULL	Limitation 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Limitation of atherosclerosis in coronary arteries with pravastatin ( PLAC 1 ) ) .
	manualset3
251598	2	425658	7	NULL	NULL	0	NULL	atherosclerosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Limitation of atherosclerosis in coronary arteries with pravastatin ( PLAC 1 ) ) .
	manualset3
251599	3	425658	7	NULL	NULL	0	NULL	coronary arteries	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Limitation of atherosclerosis in coronary arteries with pravastatin ( PLAC 1 ) ) .
	manualset3
251600	4	425658	7	NULL	NULL	0	NULL	pravastatin ( PLAC 1 ) 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Limitation of atherosclerosis in coronary arteries with pravastatin ( PLAC 1 ) ) .
	manualset3
251601	1	425659	7	NULL	NULL	0	NULL	Considerations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Considerations of tumor response kinetics and somatic mutation suggest that these biologic factors are fundamentally responsible .
	manualset3
251602	2	425659	7	NULL	NULL	0	NULL	tumor response kinetics 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Considerations of tumor response kinetics and somatic mutation suggest that these biologic factors are fundamentally responsible .
	manualset3
251603	3	425659	7	NULL	NULL	0	NULL	somatic mutation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Considerations of tumor response kinetics and somatic mutation suggest that these biologic factors are fundamentally responsible .
	manualset3
251604	4	425659	7	NULL	NULL	0	NULL	biologic factors 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Considerations of tumor response kinetics and somatic mutation suggest that these biologic factors are fundamentally responsible .
	manualset3
251605	1	425660	7	NULL	NULL	0	NULL	external calibration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering external calibration as quantification technique , the overall recoveries ( accuracy ) of the procedure ranged between 81 % and 114 % for red and white wine samples ( 10-20 mL ) , spiked at different concentrations between 5 and 100 ng mL ( -1 ) .
	manualset3
251606	2	425660	7	NULL	NULL	0	NULL	quantification technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering external calibration as quantification technique , the overall recoveries ( accuracy ) of the procedure ranged between 81 % and 114 % for red and white wine samples ( 10-20 mL ) , spiked at different concentrations between 5 and 100 ng mL ( -1 ) .
	manualset3
251607	3	425660	7	NULL	NULL	0	NULL	recoveries	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering external calibration as quantification technique , the overall recoveries ( accuracy ) of the procedure ranged between 81 % and 114 % for red and white wine samples ( 10-20 mL ) , spiked at different concentrations between 5 and 100 ng mL ( -1 ) .
	manualset3
251608	4	425660	7	NULL	NULL	0	NULL	accuracy	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering external calibration as quantification technique , the overall recoveries ( accuracy ) of the procedure ranged between 81 % and 114 % for red and white wine samples ( 10-20 mL ) , spiked at different concentrations between 5 and 100 ng mL ( -1 ) .
	manualset3
251609	5	425660	7	NULL	NULL	0	NULL	procedure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering external calibration as quantification technique , the overall recoveries ( accuracy ) of the procedure ranged between 81 % and 114 % for red and white wine samples ( 10-20 mL ) , spiked at different concentrations between 5 and 100 ng mL ( -1 ) .
	manualset3
251610	6	425660	7	NULL	NULL	0	NULL	81 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering external calibration as quantification technique , the overall recoveries ( accuracy ) of the procedure ranged between 81 % and 114 % for red and white wine samples ( 10-20 mL ) , spiked at different concentrations between 5 and 100 ng mL ( -1 ) .
	manualset3
251611	7	425660	7	NULL	NULL	0	NULL	 114 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering external calibration as quantification technique , the overall recoveries ( accuracy ) of the procedure ranged between 81 % and 114 % for red and white wine samples ( 10-20 mL ) , spiked at different concentrations between 5 and 100 ng mL ( -1 ) .
	manualset3
251612	8	425660	7	NULL	NULL	0	NULL	 red wine samples	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering external calibration as quantification technique , the overall recoveries ( accuracy ) of the procedure ranged between 81 % and 114 % for red and white wine samples ( 10-20 mL ) , spiked at different concentrations between 5 and 100 ng mL ( -1 ) .
	manualset3
251613	9	425660	7	NULL	NULL	0	NULL	white wine samples	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering external calibration as quantification technique , the overall recoveries ( accuracy ) of the procedure ranged between 81 % and 114 % for red and white wine samples ( 10-20 mL ) , spiked at different concentrations between 5 and 100 ng mL ( -1 ) .
	manualset3
251614	10	425660	7	NULL	NULL	0	NULL	10-20 mL	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering external calibration as quantification technique , the overall recoveries ( accuracy ) of the procedure ranged between 81 % and 114 % for red and white wine samples ( 10-20 mL ) , spiked at different concentrations between 5 and 100 ng mL ( -1 ) .
	manualset3
251615	11	425660	7	NULL	NULL	0	NULL	different concentrations 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering external calibration as quantification technique , the overall recoveries ( accuracy ) of the procedure ranged between 81 % and 114 % for red and white wine samples ( 10-20 mL ) , spiked at different concentrations between 5 and 100 ng mL ( -1 ) .
	manualset3
251616	12	425660	7	NULL	NULL	0	NULL	5 ng mL ( -1 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering external calibration as quantification technique , the overall recoveries ( accuracy ) of the procedure ranged between 81 % and 114 % for red and white wine samples ( 10-20 mL ) , spiked at different concentrations between 5 and 100 ng mL ( -1 ) .
	manualset3
251617	13	425660	7	NULL	NULL	0	NULL	100 ng mL ( -1 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering external calibration as quantification technique , the overall recoveries ( accuracy ) of the procedure ranged between 81 % and 114 % for red and white wine samples ( 10-20 mL ) , spiked at different concentrations between 5 and 100 ng mL ( -1 ) .
	manualset3
252122	1	425661	7	NULL	NULL	0	NULL	experience 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering our acquired experience in both laparoscopic liver resection and standard open surgery for live donation in pediatric and adult patients , we decided to offer , for the first time in Belgium , a laparoscopic approach for the left lateral sectionectomy to a young mother .
	manualset3
252123	2	425661	7	NULL	NULL	0	NULL	 laparoscopic liver resection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering our acquired experience in both laparoscopic liver resection and standard open surgery for live donation in pediatric and adult patients , we decided to offer , for the first time in Belgium , a laparoscopic approach for the left lateral sectionectomy to a young mother .
	manualset3
252128	3	425661	7	NULL	NULL	0	NULL	 standard open surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering our acquired experience in both laparoscopic liver resection and standard open surgery for live donation in pediatric and adult patients , we decided to offer , for the first time in Belgium , a laparoscopic approach for the left lateral sectionectomy to a young mother .
	manualset3
252129	4	425661	7	NULL	NULL	0	NULL	 live donation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering our acquired experience in both laparoscopic liver resection and standard open surgery for live donation in pediatric and adult patients , we decided to offer , for the first time in Belgium , a laparoscopic approach for the left lateral sectionectomy to a young mother .
	manualset3
252130	5	425661	7	NULL	NULL	0	NULL	 pediatric patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering our acquired experience in both laparoscopic liver resection and standard open surgery for live donation in pediatric and adult patients , we decided to offer , for the first time in Belgium , a laparoscopic approach for the left lateral sectionectomy to a young mother .
	manualset3
252131	6	425661	7	NULL	NULL	0	NULL	adult patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering our acquired experience in both laparoscopic liver resection and standard open surgery for live donation in pediatric and adult patients , we decided to offer , for the first time in Belgium , a laparoscopic approach for the left lateral sectionectomy to a young mother .
	manualset3
252132	7	425661	7	NULL	NULL	0	NULL	first time	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering our acquired experience in both laparoscopic liver resection and standard open surgery for live donation in pediatric and adult patients , we decided to offer , for the first time in Belgium , a laparoscopic approach for the left lateral sectionectomy to a young mother .
	manualset3
252134	8	425661	7	NULL	NULL	0	NULL	Belgium	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering our acquired experience in both laparoscopic liver resection and standard open surgery for live donation in pediatric and adult patients , we decided to offer , for the first time in Belgium , a laparoscopic approach for the left lateral sectionectomy to a young mother .
	manualset3
252135	9	425661	7	NULL	NULL	0	NULL	laparoscopic approach	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering our acquired experience in both laparoscopic liver resection and standard open surgery for live donation in pediatric and adult patients , we decided to offer , for the first time in Belgium , a laparoscopic approach for the left lateral sectionectomy to a young mother .
	manualset3
252137	10	425661	7	NULL	NULL	0	NULL	 left lateral sectionectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering our acquired experience in both laparoscopic liver resection and standard open surgery for live donation in pediatric and adult patients , we decided to offer , for the first time in Belgium , a laparoscopic approach for the left lateral sectionectomy to a young mother .
	manualset3
252138	11	425661	7	NULL	NULL	0	NULL	young mother	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering our acquired experience in both laparoscopic liver resection and standard open surgery for live donation in pediatric and adult patients , we decided to offer , for the first time in Belgium , a laparoscopic approach for the left lateral sectionectomy to a young mother .
	manualset3
252145	1	425662	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering these results and the fact that plasma half-life of clonidine at the dose administered is approximately 3h , it is possible to speculate that the inhibitory effect of clonidine on sodium appetite may be independent of - endorphin modulation during the first stage ; however , the long-lasting inhibitory effect of clonidine may be mediated by the - endorphinergic system .
	manualset3
252146	2	425662	7	NULL	NULL	0	NULL	plasma half-life	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering these results and the fact that plasma half-life of clonidine at the dose administered is approximately 3h , it is possible to speculate that the inhibitory effect of clonidine on sodium appetite may be independent of - endorphin modulation during the first stage ; however , the long-lasting inhibitory effect of clonidine may be mediated by the - endorphinergic system .
	manualset3
252147	3	425662	7	NULL	NULL	0	NULL	clonidine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering these results and the fact that plasma half-life of clonidine at the dose administered is approximately 3h , it is possible to speculate that the inhibitory effect of clonidine on sodium appetite may be independent of - endorphin modulation during the first stage ; however , the long-lasting inhibitory effect of clonidine may be mediated by the - endorphinergic system .
	manualset3
252148	4	425662	7	NULL	NULL	0	NULL	dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering these results and the fact that plasma half-life of clonidine at the dose administered is approximately 3h , it is possible to speculate that the inhibitory effect of clonidine on sodium appetite may be independent of - endorphin modulation during the first stage ; however , the long-lasting inhibitory effect of clonidine may be mediated by the - endorphinergic system .
	manualset3
252149	5	425662	7	NULL	NULL	0	NULL	 3h 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering these results and the fact that plasma half-life of clonidine at the dose administered is approximately 3h , it is possible to speculate that the inhibitory effect of clonidine on sodium appetite may be independent of - endorphin modulation during the first stage ; however , the long-lasting inhibitory effect of clonidine may be mediated by the - endorphinergic system .
	manualset3
252150	6	425662	7	NULL	NULL	0	NULL	inhibitory effect 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering these results and the fact that plasma half-life of clonidine at the dose administered is approximately 3h , it is possible to speculate that the inhibitory effect of clonidine on sodium appetite may be independent of - endorphin modulation during the first stage ; however , the long-lasting inhibitory effect of clonidine may be mediated by the - endorphinergic system .
	manualset3
252151	7	425662	7	NULL	NULL	0	NULL	clonidine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering these results and the fact that plasma half-life of clonidine at the dose administered is approximately 3h , it is possible to speculate that the inhibitory effect of clonidine on sodium appetite may be independent of - endorphin modulation during the first stage ; however , the long-lasting inhibitory effect of clonidine may be mediated by the - endorphinergic system .
	manualset3
252152	8	425662	7	NULL	NULL	0	NULL	sodium appetite	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering these results and the fact that plasma half-life of clonidine at the dose administered is approximately 3h , it is possible to speculate that the inhibitory effect of clonidine on sodium appetite may be independent of - endorphin modulation during the first stage ; however , the long-lasting inhibitory effect of clonidine may be mediated by the - endorphinergic system .
	manualset3
252153	9	425662	7	NULL	NULL	0	NULL	endorphin modulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering these results and the fact that plasma half-life of clonidine at the dose administered is approximately 3h , it is possible to speculate that the inhibitory effect of clonidine on sodium appetite may be independent of - endorphin modulation during the first stage ; however , the long-lasting inhibitory effect of clonidine may be mediated by the - endorphinergic system .
	manualset3
252154	10	425662	7	NULL	NULL	0	NULL	 first stage	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering these results and the fact that plasma half-life of clonidine at the dose administered is approximately 3h , it is possible to speculate that the inhibitory effect of clonidine on sodium appetite may be independent of - endorphin modulation during the first stage ; however , the long-lasting inhibitory effect of clonidine may be mediated by the - endorphinergic system .
	manualset3
252156	11	425662	7	NULL	NULL	0	NULL	 long-lasting inhibitory effect 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering these results and the fact that plasma half-life of clonidine at the dose administered is approximately 3h , it is possible to speculate that the inhibitory effect of clonidine on sodium appetite may be independent of - endorphin modulation during the first stage ; however , the long-lasting inhibitory effect of clonidine may be mediated by the - endorphinergic system .
	manualset3
252158	12	425662	7	NULL	NULL	0	NULL	clonidine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering these results and the fact that plasma half-life of clonidine at the dose administered is approximately 3h , it is possible to speculate that the inhibitory effect of clonidine on sodium appetite may be independent of - endorphin modulation during the first stage ; however , the long-lasting inhibitory effect of clonidine may be mediated by the - endorphinergic system .
	manualset3
252159	13	425662	7	NULL	NULL	0	NULL	endorphinergic system 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Considering these results and the fact that plasma half-life of clonidine at the dose administered is approximately 3h , it is possible to speculate that the inhibitory effect of clonidine on sodium appetite may be independent of - endorphin modulation during the first stage ; however , the long-lasting inhibitory effect of clonidine may be mediated by the - endorphinergic system .
	manualset3
252160	1	425663	7	NULL	NULL	0	NULL	minor role	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with a minor role for ATP P2 receptors on eSLEs we could detect no ATP release during eSLEs , although appreciable quantities of adenosine were detected , which had a pronounced inhibitory action on eSLEs via A ( 1 ) receptors .
	manualset3
252161	2	425663	7	NULL	NULL	0	NULL	ATP P2 receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with a minor role for ATP P2 receptors on eSLEs we could detect no ATP release during eSLEs , although appreciable quantities of adenosine were detected , which had a pronounced inhibitory action on eSLEs via A ( 1 ) receptors .
	manualset3
252162	3	425663	7	NULL	NULL	0	NULL	eSLEs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with a minor role for ATP P2 receptors on eSLEs we could detect no ATP release during eSLEs , although appreciable quantities of adenosine were detected , which had a pronounced inhibitory action on eSLEs via A ( 1 ) receptors .
	manualset3
252163	4	425663	7	NULL	NULL	0	NULL	 ATP release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with a minor role for ATP P2 receptors on eSLEs we could detect no ATP release during eSLEs , although appreciable quantities of adenosine were detected , which had a pronounced inhibitory action on eSLEs via A ( 1 ) receptors .
	manualset3
252164	5	425663	7	NULL	NULL	0	NULL	eSLEs 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with a minor role for ATP P2 receptors on eSLEs we could detect no ATP release during eSLEs , although appreciable quantities of adenosine were detected , which had a pronounced inhibitory action on eSLEs via A ( 1 ) receptors .
	manualset3
252165	6	425663	7	NULL	NULL	0	NULL	quantities	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with a minor role for ATP P2 receptors on eSLEs we could detect no ATP release during eSLEs , although appreciable quantities of adenosine were detected , which had a pronounced inhibitory action on eSLEs via A ( 1 ) receptors .
	manualset3
252166	7	425663	7	NULL	NULL	0	NULL	adenosine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with a minor role for ATP P2 receptors on eSLEs we could detect no ATP release during eSLEs , although appreciable quantities of adenosine were detected , which had a pronounced inhibitory action on eSLEs via A ( 1 ) receptors .
	manualset3
252167	8	425663	7	NULL	NULL	0	NULL	inhibitory action 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with a minor role for ATP P2 receptors on eSLEs we could detect no ATP release during eSLEs , although appreciable quantities of adenosine were detected , which had a pronounced inhibitory action on eSLEs via A ( 1 ) receptors .
	manualset3
252168	9	425663	7	NULL	NULL	0	NULL	eSLEs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with a minor role for ATP P2 receptors on eSLEs we could detect no ATP release during eSLEs , although appreciable quantities of adenosine were detected , which had a pronounced inhibitory action on eSLEs via A ( 1 ) receptors .
	manualset3
252169	10	425663	7	NULL	NULL	0	NULL	A ( 1 ) receptors	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with a minor role for ATP P2 receptors on eSLEs we could detect no ATP release during eSLEs , although appreciable quantities of adenosine were detected , which had a pronounced inhibitory action on eSLEs via A ( 1 ) receptors .
	manualset3
252170	1	425664	7	NULL	NULL	0	NULL	Limitation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Limitation of the vascular effects of noradrenaline using noradrenaline itself ) .
	manualset3
252171	2	425664	7	NULL	NULL	0	NULL	 vascular effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Limitation of the vascular effects of noradrenaline using noradrenaline itself ) .
	manualset3
252172	3	425664	7	NULL	NULL	0	NULL	noradrenaline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Limitation of the vascular effects of noradrenaline using noradrenaline itself ) .
	manualset3
252173	4	425664	7	NULL	NULL	0	NULL	 noradrenaline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Limitation of the vascular effects of noradrenaline using noradrenaline itself ) .
	manualset3
252177	1	425665	7	NULL	NULL	0	NULL	metabolic stability	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with its metabolic stability , the response elicited by the N-methylated peptide was found to be more sustained than that caused by systemin .
	manualset3
252184	2	425665	7	NULL	NULL	0	NULL	 response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with its metabolic stability , the response elicited by the N-methylated peptide was found to be more sustained than that caused by systemin .
	manualset3
252185	3	425665	7	NULL	NULL	0	NULL	N-methylated peptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with its metabolic stability , the response elicited by the N-methylated peptide was found to be more sustained than that caused by systemin .
	manualset3
252186	4	425665	7	NULL	NULL	0	NULL	systemin	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with its metabolic stability , the response elicited by the N-methylated peptide was found to be more sustained than that caused by systemin .
	manualset3
252188	1	425666	7	NULL	NULL	0	NULL	findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with previous findings , the strongest projections were observed in the superficial layers of the superior colliculus , the dorsal and ventral lateral geniculate nuclei , the pretectal nuclei , the accessory optic nuclei , and the suprachiasmatic nucleus of the hypothalamus .
	manualset3
252189	2	425666	7	NULL	NULL	0	NULL	strongest projections	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with previous findings , the strongest projections were observed in the superficial layers of the superior colliculus , the dorsal and ventral lateral geniculate nuclei , the pretectal nuclei , the accessory optic nuclei , and the suprachiasmatic nucleus of the hypothalamus .
	manualset3
252193	3	425666	7	NULL	NULL	0	NULL	superficial layers 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with previous findings , the strongest projections were observed in the superficial layers of the superior colliculus , the dorsal and ventral lateral geniculate nuclei , the pretectal nuclei , the accessory optic nuclei , and the suprachiasmatic nucleus of the hypothalamus .
	manualset3
252196	4	425666	7	NULL	NULL	0	NULL	superior colliculus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with previous findings , the strongest projections were observed in the superficial layers of the superior colliculus , the dorsal and ventral lateral geniculate nuclei , the pretectal nuclei , the accessory optic nuclei , and the suprachiasmatic nucleus of the hypothalamus .
	manualset3
252197	5	425666	7	NULL	NULL	0	NULL	 dorsal lateral geniculate nuclei	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with previous findings , the strongest projections were observed in the superficial layers of the superior colliculus , the dorsal and ventral lateral geniculate nuclei , the pretectal nuclei , the accessory optic nuclei , and the suprachiasmatic nucleus of the hypothalamus .
	manualset3
252198	6	425666	7	NULL	NULL	0	NULL	ventral lateral geniculate nuclei 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with previous findings , the strongest projections were observed in the superficial layers of the superior colliculus , the dorsal and ventral lateral geniculate nuclei , the pretectal nuclei , the accessory optic nuclei , and the suprachiasmatic nucleus of the hypothalamus .
	manualset3
252199	7	425666	7	NULL	NULL	0	NULL	pretectal nuclei	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with previous findings , the strongest projections were observed in the superficial layers of the superior colliculus , the dorsal and ventral lateral geniculate nuclei , the pretectal nuclei , the accessory optic nuclei , and the suprachiasmatic nucleus of the hypothalamus .
	manualset3
252200	8	425666	7	NULL	NULL	0	NULL	accessory optic nuclei	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with previous findings , the strongest projections were observed in the superficial layers of the superior colliculus , the dorsal and ventral lateral geniculate nuclei , the pretectal nuclei , the accessory optic nuclei , and the suprachiasmatic nucleus of the hypothalamus .
	manualset3
252201	9	425666	7	NULL	NULL	0	NULL	suprachiasmatic nucleus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with previous findings , the strongest projections were observed in the superficial layers of the superior colliculus , the dorsal and ventral lateral geniculate nuclei , the pretectal nuclei , the accessory optic nuclei , and the suprachiasmatic nucleus of the hypothalamus .
	manualset3
252202	10	425666	7	NULL	NULL	0	NULL	hypothalamus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with previous findings , the strongest projections were observed in the superficial layers of the superior colliculus , the dorsal and ventral lateral geniculate nuclei , the pretectal nuclei , the accessory optic nuclei , and the suprachiasmatic nucleus of the hypothalamus .
	manualset3
252203	1	425667	7	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with the hypothesis that this is a functional variant , KIT mRNA and protein levels are both increased in the majority of samples harboring the KIT variant .
	manualset3
252206	2	425667	7	NULL	NULL	0	NULL	functional variant 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with the hypothesis that this is a functional variant , KIT mRNA and protein levels are both increased in the majority of samples harboring the KIT variant .
	manualset3
252208	3	425667	7	NULL	NULL	0	NULL	KIT mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with the hypothesis that this is a functional variant , KIT mRNA and protein levels are both increased in the majority of samples harboring the KIT variant .
	manualset3
252210	4	425667	7	NULL	NULL	0	NULL	protein levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with the hypothesis that this is a functional variant , KIT mRNA and protein levels are both increased in the majority of samples harboring the KIT variant .
	manualset3
252211	5	425667	7	NULL	NULL	0	NULL	majority	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with the hypothesis that this is a functional variant , KIT mRNA and protein levels are both increased in the majority of samples harboring the KIT variant .
	manualset3
252212	6	425667	7	NULL	NULL	0	NULL	samples	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with the hypothesis that this is a functional variant , KIT mRNA and protein levels are both increased in the majority of samples harboring the KIT variant .
	manualset3
252213	7	425667	7	NULL	NULL	0	NULL	KIT variant 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with the hypothesis that this is a functional variant , KIT mRNA and protein levels are both increased in the majority of samples harboring the KIT variant .
	manualset3
252214	1	425668	7	NULL	NULL	0	NULL	hypothesis	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with the latter hypothesis , we show that HR events occurring in BRCA2-defective cells differ from HR events in wild-type cells .
	manualset3
252216	2	425668	7	NULL	NULL	0	NULL	HR events	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with the latter hypothesis , we show that HR events occurring in BRCA2-defective cells differ from HR events in wild-type cells .
	manualset3
252217	3	425668	7	NULL	NULL	0	NULL	BRCA2-defective cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with the latter hypothesis , we show that HR events occurring in BRCA2-defective cells differ from HR events in wild-type cells .
	manualset3
252219	4	425668	7	NULL	NULL	0	NULL	HR events	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with the latter hypothesis , we show that HR events occurring in BRCA2-defective cells differ from HR events in wild-type cells .
	manualset3
252221	5	425668	7	NULL	NULL	0	NULL	wild-type cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with the latter hypothesis , we show that HR events occurring in BRCA2-defective cells differ from HR events in wild-type cells .
	manualset3
252226	1	425669	7	NULL	NULL	0	NULL	theoretical expectations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with theoretical expectations , HBA-T1 and HBA-T2 were characterized by highly elevated levels of diversity between populations and between allele classes .
	manualset3
252236	2	425669	7	NULL	NULL	0	NULL	HBA-T1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with theoretical expectations , HBA-T1 and HBA-T2 were characterized by highly elevated levels of diversity between populations and between allele classes .
	manualset3
252237	3	425669	7	NULL	NULL	0	NULL	HBA-T2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with theoretical expectations , HBA-T1 and HBA-T2 were characterized by highly elevated levels of diversity between populations and between allele classes .
	manualset3
252238	4	425669	7	NULL	NULL	0	NULL	highly elevated levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with theoretical expectations , HBA-T1 and HBA-T2 were characterized by highly elevated levels of diversity between populations and between allele classes .
	manualset3
252239	5	425669	7	NULL	NULL	NULL	NULL	diversity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Consistent with theoretical expectations , HBA-T1 and HBA-T2 were characterized by highly elevated levels of diversity between populations and between allele classes .
	manualset3
252240	6	425669	7	NULL	NULL	0	NULL	 populations	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with theoretical expectations , HBA-T1 and HBA-T2 were characterized by highly elevated levels of diversity between populations and between allele classes .
	manualset3
252241	7	425669	7	NULL	NULL	0	NULL	allele classes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with theoretical expectations , HBA-T1 and HBA-T2 were characterized by highly elevated levels of diversity between populations and between allele classes .
	manualset3
252242	1	425670	7	NULL	NULL	0	NULL	 observations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with these observations , germ-free mice are protected from obesity and many forms of liver injury .
	manualset3
252243	2	425670	7	NULL	NULL	0	NULL	germ-free mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with these observations , germ-free mice are protected from obesity and many forms of liver injury .
	manualset3
252244	3	425670	7	NULL	NULL	0	NULL	obesity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with these observations , germ-free mice are protected from obesity and many forms of liver injury .
	manualset3
252245	4	425670	7	NULL	NULL	0	NULL	forms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with these observations , germ-free mice are protected from obesity and many forms of liver injury .
	manualset3
252246	5	425670	7	NULL	NULL	0	NULL	liver injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with these observations , germ-free mice are protected from obesity and many forms of liver injury .
	manualset3
252247	1	425671	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with these results , TcrPDEC2 localizes to the contractile vacuole complex , showing strong labeling in the region corresponding to the spongiome .
	manualset3
252248	2	425671	7	NULL	NULL	0	NULL	 TcrPDEC2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with these results , TcrPDEC2 localizes to the contractile vacuole complex , showing strong labeling in the region corresponding to the spongiome .
	manualset3
252249	3	425671	7	NULL	NULL	0	NULL	contractile vacuole complex	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with these results , TcrPDEC2 localizes to the contractile vacuole complex , showing strong labeling in the region corresponding to the spongiome .
	manualset3
252250	4	425671	7	NULL	NULL	0	NULL	 strong labeling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with these results , TcrPDEC2 localizes to the contractile vacuole complex , showing strong labeling in the region corresponding to the spongiome .
	manualset3
252251	5	425671	7	NULL	NULL	0	NULL	 region	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with these results , TcrPDEC2 localizes to the contractile vacuole complex , showing strong labeling in the region corresponding to the spongiome .
	manualset3
252252	6	425671	7	NULL	NULL	0	NULL	spongiome	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with these results , TcrPDEC2 localizes to the contractile vacuole complex , showing strong labeling in the region corresponding to the spongiome .
	manualset3
252253	1	425672	7	NULL	NULL	0	NULL	 results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with these results , an enforced expression of the miR-221 and miR-222 induced the thyroid papillary carcinoma cell line ( TPC-1 ) to progress to the S phase of the cell cycle .
	manualset3
252254	2	425672	7	NULL	NULL	0	NULL	enforced expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with these results , an enforced expression of the miR-221 and miR-222 induced the thyroid papillary carcinoma cell line ( TPC-1 ) to progress to the S phase of the cell cycle .
	manualset3
252255	3	425672	7	NULL	NULL	0	NULL	 miR-221	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with these results , an enforced expression of the miR-221 and miR-222 induced the thyroid papillary carcinoma cell line ( TPC-1 ) to progress to the S phase of the cell cycle .
	manualset3
252256	4	425672	7	NULL	NULL	0	NULL	miR-222	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with these results , an enforced expression of the miR-221 and miR-222 induced the thyroid papillary carcinoma cell line ( TPC-1 ) to progress to the S phase of the cell cycle .
	manualset3
252257	5	425672	7	NULL	NULL	0	NULL	thyroid papillary carcinoma cell line ( TPC-1 )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with these results , an enforced expression of the miR-221 and miR-222 induced the thyroid papillary carcinoma cell line ( TPC-1 ) to progress to the S phase of the cell cycle .
	manualset3
252258	6	425672	7	NULL	NULL	0	NULL	 S phase	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with these results , an enforced expression of the miR-221 and miR-222 induced the thyroid papillary carcinoma cell line ( TPC-1 ) to progress to the S phase of the cell cycle .
	manualset3
252259	7	425672	7	NULL	NULL	0	NULL	 cell cycle	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with these results , an enforced expression of the miR-221 and miR-222 induced the thyroid papillary carcinoma cell line ( TPC-1 ) to progress to the S phase of the cell cycle .
	manualset3
252260	1	425673	7	NULL	NULL	0	NULL	 increase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with this , we detected an increase in ICAM and VCAM , both indicators of endothelial activation , a known trigger for secretion of S100A8 and S100A9 .
	manualset3
252261	2	425673	7	NULL	NULL	0	NULL	 ICAM 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with this , we detected an increase in ICAM and VCAM , both indicators of endothelial activation , a known trigger for secretion of S100A8 and S100A9 .
	manualset3
252262	3	425673	7	NULL	NULL	0	NULL	VCAM	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with this , we detected an increase in ICAM and VCAM , both indicators of endothelial activation , a known trigger for secretion of S100A8 and S100A9 .
	manualset3
252263	4	425673	7	NULL	NULL	0	NULL	indicators	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with this , we detected an increase in ICAM and VCAM , both indicators of endothelial activation , a known trigger for secretion of S100A8 and S100A9 .
	manualset3
252264	5	425673	7	NULL	NULL	0	NULL	endothelial activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with this , we detected an increase in ICAM and VCAM , both indicators of endothelial activation , a known trigger for secretion of S100A8 and S100A9 .
	manualset3
252265	6	425673	7	NULL	NULL	0	NULL	trigger	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with this , we detected an increase in ICAM and VCAM , both indicators of endothelial activation , a known trigger for secretion of S100A8 and S100A9 .
	manualset3
252266	7	425673	7	NULL	NULL	NULL	NULL	secretion 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Consistent with this , we detected an increase in ICAM and VCAM , both indicators of endothelial activation , a known trigger for secretion of S100A8 and S100A9 .
	manualset3
252267	8	425673	7	NULL	NULL	0	NULL	S100A8 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with this , we detected an increase in ICAM and VCAM , both indicators of endothelial activation , a known trigger for secretion of S100A8 and S100A9 .
	manualset3
252268	9	425673	7	NULL	NULL	0	NULL	S100A9	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with this , we detected an increase in ICAM and VCAM , both indicators of endothelial activation , a known trigger for secretion of S100A8 and S100A9 .
	manualset3
252269	1	425674	7	NULL	NULL	0	NULL	finding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with this finding , immunoblotting revealed that this cotreatment significantly increased expression of phosphorylated AQP2 .
	manualset3
252270	2	425674	7	NULL	NULL	0	NULL	 immunoblotting	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with this finding , immunoblotting revealed that this cotreatment significantly increased expression of phosphorylated AQP2 .
	manualset3
252271	3	425674	7	NULL	NULL	0	NULL	cotreatment 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with this finding , immunoblotting revealed that this cotreatment significantly increased expression of phosphorylated AQP2 .
	manualset3
252272	4	425674	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with this finding , immunoblotting revealed that this cotreatment significantly increased expression of phosphorylated AQP2 .
	manualset3
252273	5	425674	7	NULL	NULL	0	NULL	 phosphorylated AQP2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistent with this finding , immunoblotting revealed that this cotreatment significantly increased expression of phosphorylated AQP2 .
	manualset3
252274	1	425675	7	NULL	NULL	0	NULL	 study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( A study of correlation between the change of chromosome centromeric dots and habitual abortions ) .
	manualset3
252275	2	425675	7	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	( A study of correlation between the change of chromosome centromeric dots and habitual abortions ) .
	manualset3
252276	3	425675	7	NULL	NULL	0	NULL	change	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( A study of correlation between the change of chromosome centromeric dots and habitual abortions ) .
	manualset3
252277	4	425675	7	NULL	NULL	0	NULL	chromosome centromeric dots	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	( A study of correlation between the change of chromosome centromeric dots and habitual abortions ) .
	manualset3
252278	5	425675	7	NULL	NULL	0	NULL	habitual abortions 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( A study of correlation between the change of chromosome centromeric dots and habitual abortions ) .
	manualset3
252279	1	425676	7	NULL	NULL	0	NULL	 Limits	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Limits of efficacy and tolerance of antidepressive medications ) .
	manualset3
252280	2	425676	7	NULL	NULL	NULL	NULL	tolerance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Limits of efficacy and tolerance of antidepressive medications ) .
	manualset3
252281	3	425676	7	NULL	NULL	0	NULL	antidepressive medications	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Limits of efficacy and tolerance of antidepressive medications ) .
	manualset3
254245	4	425676	7	NULL	NULL	NULL	NULL	efficacy	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Limits of efficacy and tolerance of antidepressive medications ) .
	manualset3
252282	1	425677	7	NULL	NULL	0	NULL	DATS treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistently , DATS treatment leads to the induction of the skn-1 target gene gst-4 , and this induction was dependent on skn-1 .
	manualset3
252283	2	425677	7	NULL	NULL	0	NULL	induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistently , DATS treatment leads to the induction of the skn-1 target gene gst-4 , and this induction was dependent on skn-1 .
	manualset3
252284	3	425677	7	NULL	NULL	0	NULL	skn-1 target gene gst-4	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistently , DATS treatment leads to the induction of the skn-1 target gene gst-4 , and this induction was dependent on skn-1 .
	manualset3
252285	4	425677	7	NULL	NULL	0	NULL	induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistently , DATS treatment leads to the induction of the skn-1 target gene gst-4 , and this induction was dependent on skn-1 .
	manualset3
252286	5	425677	7	NULL	NULL	0	NULL	 skn-1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistently , DATS treatment leads to the induction of the skn-1 target gene gst-4 , and this induction was dependent on skn-1 .
	manualset3
252287	1	425678	7	NULL	NULL	0	NULL	two Tup proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistently , we show that the two Tup proteins can interact together when expressed at normal levels and that each can independently interact with the Ssn6 protein , as seen for Tup1 in budding yeast .
	manualset3
252288	2	425678	7	NULL	NULL	0	NULL	normal levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistently , we show that the two Tup proteins can interact together when expressed at normal levels and that each can independently interact with the Ssn6 protein , as seen for Tup1 in budding yeast .
	manualset3
252289	3	425678	7	NULL	NULL	0	NULL	Ssn6 protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistently , we show that the two Tup proteins can interact together when expressed at normal levels and that each can independently interact with the Ssn6 protein , as seen for Tup1 in budding yeast .
	manualset3
252290	4	425678	7	NULL	NULL	0	NULL	Tup1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistently , we show that the two Tup proteins can interact together when expressed at normal levels and that each can independently interact with the Ssn6 protein , as seen for Tup1 in budding yeast .
	manualset3
252291	5	425678	7	NULL	NULL	0	NULL	budding yeast	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Consistently , we show that the two Tup proteins can interact together when expressed at normal levels and that each can independently interact with the Ssn6 protein , as seen for Tup1 in budding yeast .
	manualset3
252292	1	425679	7	NULL	NULL	0	NULL	 negative density	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Conspecific negative density dependence and forest diversity .
	manualset3
252293	2	425679	7	NULL	NULL	0	NULL	forest diversity	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Conspecific negative density dependence and forest diversity .
	manualset3
252294	1	425680	7	NULL	NULL	0	NULL	Constitutive ERK MAPK activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Constitutive ERK MAPK activity regulates macrophage ATP production and mitochondrial integrity .
	manualset3
252295	2	425680	7	NULL	NULL	0	NULL	 macrophage ATP production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Constitutive ERK MAPK activity regulates macrophage ATP production and mitochondrial integrity .
	manualset3
252296	3	425680	7	NULL	NULL	0	NULL	mitochondrial integrity 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Constitutive ERK MAPK activity regulates macrophage ATP production and mitochondrial integrity .
	manualset3
252297	1	425681	7	NULL	NULL	0	NULL	Constitutive production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Constitutive production of tat22 by Jurkat T cells in the context of both vectors blocked HIV-1 replication during lytic infection .
	manualset3
252298	2	425681	7	NULL	NULL	0	NULL	tat22 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Constitutive production of tat22 by Jurkat T cells in the context of both vectors blocked HIV-1 replication during lytic infection .
	manualset3
252299	3	425681	7	NULL	NULL	0	NULL	Jurkat T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Constitutive production of tat22 by Jurkat T cells in the context of both vectors blocked HIV-1 replication during lytic infection .
	manualset3
252300	4	425681	7	NULL	NULL	0	NULL	 context	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Constitutive production of tat22 by Jurkat T cells in the context of both vectors blocked HIV-1 replication during lytic infection .
	manualset3
252301	5	425681	7	NULL	NULL	NULL	NULL	 vectors	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Constitutive production of tat22 by Jurkat T cells in the context of both vectors blocked HIV-1 replication during lytic infection .
	manualset3
252302	6	425681	7	NULL	NULL	0	NULL	HIV-1 replication	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Constitutive production of tat22 by Jurkat T cells in the context of both vectors blocked HIV-1 replication during lytic infection .
	manualset3
252303	7	425681	7	NULL	NULL	0	NULL	lytic infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Constitutive production of tat22 by Jurkat T cells in the context of both vectors blocked HIV-1 replication during lytic infection .
	manualset3
252304	1	425682	7	NULL	NULL	0	NULL	Constitutively active Lck-Akt1 transgenes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Constitutively active Lck-Akt1 transgenes had the opposite effects .
	manualset3
252305	2	425682	7	NULL	NULL	0	NULL	 opposite effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Constitutively active Lck-Akt1 transgenes had the opposite effects .
	manualset3
252306	1	425683	7	NULL	NULL	0	NULL	Constrained dansyl derivatives	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Constrained dansyl derivatives reveal bacterial specificity of highly conserved thymidylate synthases .
	manualset3
252307	2	425683	7	NULL	NULL	0	NULL	bacterial specificity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Constrained dansyl derivatives reveal bacterial specificity of highly conserved thymidylate synthases .
	manualset3
252308	3	425683	7	NULL	NULL	0	NULL	highly conserved thymidylate synthases	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Constrained dansyl derivatives reveal bacterial specificity of highly conserved thymidylate synthases .
	manualset3
252309	1	425684	7	NULL	NULL	0	NULL	 Lipid analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Lipid and ipoprotein analysis -- clinical chemical overview -- indication for lipid analysis ) .
	manualset3
252310	2	425684	7	NULL	NULL	0	NULL	ipoprotein analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Lipid and ipoprotein analysis -- clinical chemical overview -- indication for lipid analysis ) .
	manualset3
252311	3	425684	7	NULL	NULL	0	NULL	clinical chemical overview	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Lipid and ipoprotein analysis -- clinical chemical overview -- indication for lipid analysis ) .
	manualset3
252312	4	425684	7	NULL	NULL	0	NULL	 indication	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Lipid and ipoprotein analysis -- clinical chemical overview -- indication for lipid analysis ) .
	manualset3
252313	5	425684	7	NULL	NULL	0	NULL	 lipid analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Lipid and ipoprotein analysis -- clinical chemical overview -- indication for lipid analysis ) .
	manualset3
252314	1	425685	7	NULL	NULL	0	NULL	Construction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Construction , expression and functional analysis of a glycolipid-linked form of CR1 .
	manualset3
252315	2	425685	7	NULL	NULL	NULL	NULL	expression	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Construction , expression and functional analysis of a glycolipid-linked form of CR1 .
	manualset3
252316	3	425685	7	NULL	NULL	NULL	NULL	functional analysis	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Construction , expression and functional analysis of a glycolipid-linked form of CR1 .
	manualset3
252317	4	425685	7	NULL	NULL	0	NULL	glycolipid-linked form 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Construction , expression and functional analysis of a glycolipid-linked form of CR1 .
	manualset3
252318	5	425685	7	NULL	NULL	0	NULL	 CR1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Construction , expression and functional analysis of a glycolipid-linked form of CR1 .
	manualset3
252319	1	425686	7	NULL	NULL	0	NULL	Construction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Construction of a differentiated human hepatocyte cell line expressing the herpes simplex virus-thymidine kinase gene .
	manualset3
252320	2	425686	7	NULL	NULL	0	NULL	differentiated human hepatocyte cell line	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Construction of a differentiated human hepatocyte cell line expressing the herpes simplex virus-thymidine kinase gene .
	manualset3
252321	3	425686	7	NULL	NULL	0	NULL	 herpes simplex virus-thymidine kinase gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Construction of a differentiated human hepatocyte cell line expressing the herpes simplex virus-thymidine kinase gene .
	manualset3
252322	1	425687	7	NULL	NULL	0	NULL	Construction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Construction of a tracheal pouch in rabbits .
	manualset3
252323	2	425687	7	NULL	NULL	0	NULL	tracheal pouch	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Construction of a tracheal pouch in rabbits .
	manualset3
252324	3	425687	7	NULL	NULL	0	NULL	rabbits	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Construction of a tracheal pouch in rabbits .
	manualset3
252325	1	425688	7	NULL	NULL	0	NULL	Contact hypersensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Contact hypersensitivity to picryl chloride in the mouse is proposed as a valuable tool for the in vivo immunotoxicological testing of new compounds .
	manualset3
252326	2	425688	7	NULL	NULL	0	NULL	picryl chloride	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Contact hypersensitivity to picryl chloride in the mouse is proposed as a valuable tool for the in vivo immunotoxicological testing of new compounds .
	manualset3
252327	3	425688	7	NULL	NULL	0	NULL	mouse	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Contact hypersensitivity to picryl chloride in the mouse is proposed as a valuable tool for the in vivo immunotoxicological testing of new compounds .
	manualset3
252328	4	425688	7	NULL	NULL	0	NULL	valuable tool 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Contact hypersensitivity to picryl chloride in the mouse is proposed as a valuable tool for the in vivo immunotoxicological testing of new compounds .
	manualset3
252329	5	425688	7	NULL	NULL	0	NULL	in vivo immunotoxicological testing 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Contact hypersensitivity to picryl chloride in the mouse is proposed as a valuable tool for the in vivo immunotoxicological testing of new compounds .
	manualset3
252330	6	425688	7	NULL	NULL	0	NULL	new compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Contact hypersensitivity to picryl chloride in the mouse is proposed as a valuable tool for the in vivo immunotoxicological testing of new compounds .
	manualset3
252331	1	425689	7	NULL	NULL	0	NULL	Contact laser probes	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Contact laser probes may have advantages over non-contact laser techniques for the endoscopic treatment of early gastric cancer in patients who are unfit for major surgery .
	manualset3
252332	2	425689	7	NULL	NULL	0	NULL	non-contact laser techniques	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Contact laser probes may have advantages over non-contact laser techniques for the endoscopic treatment of early gastric cancer in patients who are unfit for major surgery .
	manualset3
252333	3	425689	7	NULL	NULL	0	NULL	endoscopic treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Contact laser probes may have advantages over non-contact laser techniques for the endoscopic treatment of early gastric cancer in patients who are unfit for major surgery .
	manualset3
252334	4	425689	7	NULL	NULL	0	NULL	early gastric cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Contact laser probes may have advantages over non-contact laser techniques for the endoscopic treatment of early gastric cancer in patients who are unfit for major surgery .
	manualset3
252335	5	425689	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Contact laser probes may have advantages over non-contact laser techniques for the endoscopic treatment of early gastric cancer in patients who are unfit for major surgery .
	manualset3
252336	6	425689	7	NULL	NULL	0	NULL	major surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Contact laser probes may have advantages over non-contact laser techniques for the endoscopic treatment of early gastric cancer in patients who are unfit for major surgery .
	manualset3
252337	1	425690	7	NULL	NULL	0	NULL	Contemporary QOL questionnaires	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Contemporary QOL questionnaires are completed by patients , and they most commonly include dimensions of physical function , mental or cognitive function , emotional or psychological function , social and role function , disease symptoms , and perceptions of well-being .
	manualset3
252338	2	425690	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Contemporary QOL questionnaires are completed by patients , and they most commonly include dimensions of physical function , mental or cognitive function , emotional or psychological function , social and role function , disease symptoms , and perceptions of well-being .
	manualset3
252339	3	425690	7	NULL	NULL	0	NULL	 dimensions	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Contemporary QOL questionnaires are completed by patients , and they most commonly include dimensions of physical function , mental or cognitive function , emotional or psychological function , social and role function , disease symptoms , and perceptions of well-being .
	manualset3
252340	4	425690	7	NULL	NULL	0	NULL	physical function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contemporary QOL questionnaires are completed by patients , and they most commonly include dimensions of physical function , mental or cognitive function , emotional or psychological function , social and role function , disease symptoms , and perceptions of well-being .
	manualset3
252341	5	425690	7	NULL	NULL	0	NULL	 mental function	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contemporary QOL questionnaires are completed by patients , and they most commonly include dimensions of physical function , mental or cognitive function , emotional or psychological function , social and role function , disease symptoms , and perceptions of well-being .
	manualset3
252342	6	425690	7	NULL	NULL	0	NULL	cognitive function	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contemporary QOL questionnaires are completed by patients , and they most commonly include dimensions of physical function , mental or cognitive function , emotional or psychological function , social and role function , disease symptoms , and perceptions of well-being .
	manualset3
252343	7	425690	7	NULL	NULL	0	NULL	 emotional function	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contemporary QOL questionnaires are completed by patients , and they most commonly include dimensions of physical function , mental or cognitive function , emotional or psychological function , social and role function , disease symptoms , and perceptions of well-being .
	manualset3
252344	8	425690	7	NULL	NULL	0	NULL	psychological function	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contemporary QOL questionnaires are completed by patients , and they most commonly include dimensions of physical function , mental or cognitive function , emotional or psychological function , social and role function , disease symptoms , and perceptions of well-being .
	manualset3
252345	9	425690	7	NULL	NULL	0	NULL	 social function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contemporary QOL questionnaires are completed by patients , and they most commonly include dimensions of physical function , mental or cognitive function , emotional or psychological function , social and role function , disease symptoms , and perceptions of well-being .
	manualset3
252346	10	425690	7	NULL	NULL	0	NULL	 role function	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contemporary QOL questionnaires are completed by patients , and they most commonly include dimensions of physical function , mental or cognitive function , emotional or psychological function , social and role function , disease symptoms , and perceptions of well-being .
	manualset3
252347	11	425690	7	NULL	NULL	0	NULL	disease symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Contemporary QOL questionnaires are completed by patients , and they most commonly include dimensions of physical function , mental or cognitive function , emotional or psychological function , social and role function , disease symptoms , and perceptions of well-being .
	manualset3
252348	12	425690	7	NULL	NULL	0	NULL	perceptions 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contemporary QOL questionnaires are completed by patients , and they most commonly include dimensions of physical function , mental or cognitive function , emotional or psychological function , social and role function , disease symptoms , and perceptions of well-being .
	manualset3
252349	13	425690	7	NULL	NULL	0	NULL	well-being	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Contemporary QOL questionnaires are completed by patients , and they most commonly include dimensions of physical function , mental or cognitive function , emotional or psychological function , social and role function , disease symptoms , and perceptions of well-being .
	manualset3
252350	1	425691	7	NULL	NULL	0	NULL	Contemporary Western diets	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Contemporary Western diets yield a daily systemic acid load of varying amounts , yet the association with hypertension has never been explored .
	manualset3
252351	2	425691	7	NULL	NULL	0	NULL	daily systemic acid load	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Contemporary Western diets yield a daily systemic acid load of varying amounts , yet the association with hypertension has never been explored .
	manualset3
252352	3	425691	7	NULL	NULL	0	NULL	varying amounts	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Contemporary Western diets yield a daily systemic acid load of varying amounts , yet the association with hypertension has never been explored .
	manualset3
252353	4	425691	7	NULL	NULL	0	NULL	 association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Contemporary Western diets yield a daily systemic acid load of varying amounts , yet the association with hypertension has never been explored .
	manualset3
252354	5	425691	7	NULL	NULL	0	NULL	hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Contemporary Western diets yield a daily systemic acid load of varying amounts , yet the association with hypertension has never been explored .
	manualset3
252355	1	425692	7	NULL	NULL	0	NULL	Context effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Context effects on the neural correlates of recognition memory : an electrophysiological study .
	manualset3
252356	2	425692	7	NULL	NULL	0	NULL	 neural correlates	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Context effects on the neural correlates of recognition memory : an electrophysiological study .
	manualset3
252357	3	425692	7	NULL	NULL	0	NULL	recognition memory	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Context effects on the neural correlates of recognition memory : an electrophysiological study .
	manualset3
252358	4	425692	7	NULL	NULL	0	NULL	electrophysiological study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Context effects on the neural correlates of recognition memory : an electrophysiological study .
	manualset3
252359	1	425693	7	NULL	NULL	NULL	NULL	 Lipoprotein ( a ) 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Lipoprotein ( a ) , D-Dimer and apolipoprotein A1 as markers of presence and severity of coronary disease ) .
	manualset3
252360	2	425693	7	NULL	NULL	0	NULL	D-Dimer	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Lipoprotein ( a ) , D-Dimer and apolipoprotein A1 as markers of presence and severity of coronary disease ) .
	manualset3
252361	3	425693	7	NULL	NULL	0	NULL	apolipoprotein A1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Lipoprotein ( a ) , D-Dimer and apolipoprotein A1 as markers of presence and severity of coronary disease ) .
	manualset3
252362	4	425693	7	NULL	NULL	NULL	NULL	 markers	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Lipoprotein ( a ) , D-Dimer and apolipoprotein A1 as markers of presence and severity of coronary disease ) .
	manualset3
252363	5	425693	7	NULL	NULL	0	NULL	severity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Lipoprotein ( a ) , D-Dimer and apolipoprotein A1 as markers of presence and severity of coronary disease ) .
	manualset3
252364	6	425693	7	NULL	NULL	0	NULL	coronary disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Lipoprotein ( a ) , D-Dimer and apolipoprotein A1 as markers of presence and severity of coronary disease ) .
	manualset3
254253	7	425693	7	NULL	NULL	NULL	NULL	presence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Lipoprotein ( a ) , D-Dimer and apolipoprotein A1 as markers of presence and severity of coronary disease ) .
	manualset3
252365	1	425694	7	NULL	NULL	0	NULL	Context 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Context : Acute rheumatic fever ( ARF ) / rheumatic heart disease ( RHD ) is a major cause of morbidity and mortality in India , yet , few studies are available on susceptibility markers .
	manualset3
252366	2	425694	7	NULL	NULL	0	NULL	Acute rheumatic fever ( ARF )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Context : Acute rheumatic fever ( ARF ) / rheumatic heart disease ( RHD ) is a major cause of morbidity and mortality in India , yet , few studies are available on susceptibility markers .
	manualset3
252367	3	425694	7	NULL	NULL	0	NULL	 rheumatic heart disease ( RHD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Context : Acute rheumatic fever ( ARF ) / rheumatic heart disease ( RHD ) is a major cause of morbidity and mortality in India , yet , few studies are available on susceptibility markers .
	manualset3
252368	4	425694	7	NULL	NULL	0	NULL	 cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Context : Acute rheumatic fever ( ARF ) / rheumatic heart disease ( RHD ) is a major cause of morbidity and mortality in India , yet , few studies are available on susceptibility markers .
	manualset3
252369	5	425694	7	NULL	NULL	0	NULL	morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Context : Acute rheumatic fever ( ARF ) / rheumatic heart disease ( RHD ) is a major cause of morbidity and mortality in India , yet , few studies are available on susceptibility markers .
	manualset3
252370	6	425694	7	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Context : Acute rheumatic fever ( ARF ) / rheumatic heart disease ( RHD ) is a major cause of morbidity and mortality in India , yet , few studies are available on susceptibility markers .
	manualset3
252371	7	425694	7	NULL	NULL	0	NULL	 India	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Context : Acute rheumatic fever ( ARF ) / rheumatic heart disease ( RHD ) is a major cause of morbidity and mortality in India , yet , few studies are available on susceptibility markers .
	manualset3
252372	8	425694	7	NULL	NULL	0	NULL	studies 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Context : Acute rheumatic fever ( ARF ) / rheumatic heart disease ( RHD ) is a major cause of morbidity and mortality in India , yet , few studies are available on susceptibility markers .
	manualset3
252373	9	425694	7	NULL	NULL	0	NULL	 susceptibility markers 	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Context : Acute rheumatic fever ( ARF ) / rheumatic heart disease ( RHD ) is a major cause of morbidity and mortality in India , yet , few studies are available on susceptibility markers .
	manualset3
252374	1	425695	7	NULL	NULL	0	NULL	Context 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Context : Experimental studies linked gestational diabetes mellitus ( GDM ) and intrauterine growth restriction ( IUGR ) with altered expression of the offspring 's hypothalamic galanin mRNA , possibly contributing to the development of obesity and metabolic syndrome in later life .
	manualset3
252375	2	425695	7	NULL	NULL	0	NULL	Experimental studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Context : Experimental studies linked gestational diabetes mellitus ( GDM ) and intrauterine growth restriction ( IUGR ) with altered expression of the offspring 's hypothalamic galanin mRNA , possibly contributing to the development of obesity and metabolic syndrome in later life .
	manualset3
252376	3	425695	7	NULL	NULL	0	NULL	gestational diabetes mellitus ( GDM )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Context : Experimental studies linked gestational diabetes mellitus ( GDM ) and intrauterine growth restriction ( IUGR ) with altered expression of the offspring 's hypothalamic galanin mRNA , possibly contributing to the development of obesity and metabolic syndrome in later life .
	manualset3
252377	4	425695	7	NULL	NULL	0	NULL	intrauterine growth restriction ( IUGR )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Context : Experimental studies linked gestational diabetes mellitus ( GDM ) and intrauterine growth restriction ( IUGR ) with altered expression of the offspring 's hypothalamic galanin mRNA , possibly contributing to the development of obesity and metabolic syndrome in later life .
	manualset3
252378	5	425695	7	NULL	NULL	0	NULL	altered expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Context : Experimental studies linked gestational diabetes mellitus ( GDM ) and intrauterine growth restriction ( IUGR ) with altered expression of the offspring 's hypothalamic galanin mRNA , possibly contributing to the development of obesity and metabolic syndrome in later life .
	manualset3
252379	6	425695	7	NULL	NULL	0	NULL	 offspring 's hypothalamic galanin mRNA 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Context : Experimental studies linked gestational diabetes mellitus ( GDM ) and intrauterine growth restriction ( IUGR ) with altered expression of the offspring 's hypothalamic galanin mRNA , possibly contributing to the development of obesity and metabolic syndrome in later life .
	manualset3
252380	7	425695	7	NULL	NULL	0	NULL	 development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Context : Experimental studies linked gestational diabetes mellitus ( GDM ) and intrauterine growth restriction ( IUGR ) with altered expression of the offspring 's hypothalamic galanin mRNA , possibly contributing to the development of obesity and metabolic syndrome in later life .
	manualset3
252381	8	425695	7	NULL	NULL	0	NULL	obesity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Context : Experimental studies linked gestational diabetes mellitus ( GDM ) and intrauterine growth restriction ( IUGR ) with altered expression of the offspring 's hypothalamic galanin mRNA , possibly contributing to the development of obesity and metabolic syndrome in later life .
	manualset3
252382	9	425695	7	NULL	NULL	0	NULL	metabolic syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Context : Experimental studies linked gestational diabetes mellitus ( GDM ) and intrauterine growth restriction ( IUGR ) with altered expression of the offspring 's hypothalamic galanin mRNA , possibly contributing to the development of obesity and metabolic syndrome in later life .
	manualset3
252383	10	425695	7	NULL	NULL	0	NULL	 life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Context : Experimental studies linked gestational diabetes mellitus ( GDM ) and intrauterine growth restriction ( IUGR ) with altered expression of the offspring 's hypothalamic galanin mRNA , possibly contributing to the development of obesity and metabolic syndrome in later life .
	manualset3
252384	1	425696	7	NULL	NULL	0	NULL	Context	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Context : Low testosterone is associated with all-cause mortality , but the relationship with cause-specific mortality is uncertain .
	manualset3
252385	2	425696	7	NULL	NULL	0	NULL	Low testosterone 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Context : Low testosterone is associated with all-cause mortality , but the relationship with cause-specific mortality is uncertain .
	manualset3
252386	3	425696	7	NULL	NULL	0	NULL	all-cause mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Context : Low testosterone is associated with all-cause mortality , but the relationship with cause-specific mortality is uncertain .
	manualset3
252387	4	425696	7	NULL	NULL	0	NULL	 relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Context : Low testosterone is associated with all-cause mortality , but the relationship with cause-specific mortality is uncertain .
	manualset3
252388	5	425696	7	NULL	NULL	0	NULL	 cause-specific mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Context : Low testosterone is associated with all-cause mortality , but the relationship with cause-specific mortality is uncertain .
	manualset3
252389	1	425697	7	NULL	NULL	0	NULL	Contextual fear conditioning 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contextual fear conditioning was measured 24 h after training , and tone fear conditioning 48 h after training .
	manualset3
252390	2	425697	7	NULL	NULL	0	NULL	24 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Contextual fear conditioning was measured 24 h after training , and tone fear conditioning 48 h after training .
	manualset3
252391	3	425697	7	NULL	NULL	0	NULL	 training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contextual fear conditioning was measured 24 h after training , and tone fear conditioning 48 h after training .
	manualset3
252392	4	425697	7	NULL	NULL	0	NULL	tone fear conditioning	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contextual fear conditioning was measured 24 h after training , and tone fear conditioning 48 h after training .
	manualset3
252393	5	425697	7	NULL	NULL	0	NULL	48 h 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Contextual fear conditioning was measured 24 h after training , and tone fear conditioning 48 h after training .
	manualset3
252394	6	425697	7	NULL	NULL	0	NULL	training	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contextual fear conditioning was measured 24 h after training , and tone fear conditioning 48 h after training .
	manualset3
252395	1	425698	7	NULL	NULL	0	NULL	Continuation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuation of the national trend toward deinstitutionalization and community placement for persons with developmental disabilities , physical handicaps and other medical problems will mean increased demand for dentists trained to care for this segment of the population .
	manualset3
252396	2	425698	7	NULL	NULL	0	NULL	national trend	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuation of the national trend toward deinstitutionalization and community placement for persons with developmental disabilities , physical handicaps and other medical problems will mean increased demand for dentists trained to care for this segment of the population .
	manualset3
252397	3	425698	7	NULL	NULL	0	NULL	 deinstitutionalization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuation of the national trend toward deinstitutionalization and community placement for persons with developmental disabilities , physical handicaps and other medical problems will mean increased demand for dentists trained to care for this segment of the population .
	manualset3
252398	4	425698	7	NULL	NULL	0	NULL	community placement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuation of the national trend toward deinstitutionalization and community placement for persons with developmental disabilities , physical handicaps and other medical problems will mean increased demand for dentists trained to care for this segment of the population .
	manualset3
252399	5	425698	7	NULL	NULL	0	NULL	persons	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuation of the national trend toward deinstitutionalization and community placement for persons with developmental disabilities , physical handicaps and other medical problems will mean increased demand for dentists trained to care for this segment of the population .
	manualset3
252400	6	425698	7	NULL	NULL	0	NULL	developmental disabilities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuation of the national trend toward deinstitutionalization and community placement for persons with developmental disabilities , physical handicaps and other medical problems will mean increased demand for dentists trained to care for this segment of the population .
	manualset3
252401	7	425698	7	NULL	NULL	0	NULL	physical handicaps	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuation of the national trend toward deinstitutionalization and community placement for persons with developmental disabilities , physical handicaps and other medical problems will mean increased demand for dentists trained to care for this segment of the population .
	manualset3
252402	8	425698	7	NULL	NULL	0	NULL	medical problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuation of the national trend toward deinstitutionalization and community placement for persons with developmental disabilities , physical handicaps and other medical problems will mean increased demand for dentists trained to care for this segment of the population .
	manualset3
252403	9	425698	7	NULL	NULL	0	NULL	demand	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuation of the national trend toward deinstitutionalization and community placement for persons with developmental disabilities , physical handicaps and other medical problems will mean increased demand for dentists trained to care for this segment of the population .
	manualset3
252404	10	425698	7	NULL	NULL	0	NULL	dentists	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuation of the national trend toward deinstitutionalization and community placement for persons with developmental disabilities , physical handicaps and other medical problems will mean increased demand for dentists trained to care for this segment of the population .
	manualset3
252405	11	425698	7	NULL	NULL	0	NULL	segment	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuation of the national trend toward deinstitutionalization and community placement for persons with developmental disabilities , physical handicaps and other medical problems will mean increased demand for dentists trained to care for this segment of the population .
	manualset3
252406	12	425698	7	NULL	NULL	0	NULL	population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuation of the national trend toward deinstitutionalization and community placement for persons with developmental disabilities , physical handicaps and other medical problems will mean increased demand for dentists trained to care for this segment of the population .
	manualset3
252407	1	425699	7	NULL	NULL	0	NULL	Continuous fluorometric assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuous fluorometric assays for acetylcholinesterase activity and inhibition with conjugated polyelectrolytes .
	manualset3
252408	2	425699	7	NULL	NULL	0	NULL	acetylcholinesterase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuous fluorometric assays for acetylcholinesterase activity and inhibition with conjugated polyelectrolytes .
	manualset3
252409	3	425699	7	NULL	NULL	0	NULL	inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuous fluorometric assays for acetylcholinesterase activity and inhibition with conjugated polyelectrolytes .
	manualset3
252410	4	425699	7	NULL	NULL	0	NULL	conjugated polyelectrolytes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuous fluorometric assays for acetylcholinesterase activity and inhibition with conjugated polyelectrolytes .
	manualset3
252411	1	425700	7	NULL	NULL	0	NULL	Continuous frequency tuning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuous frequency tuning of a transversely excited CO ( 2 ) laser was achieved for the 10-microm R branch with conventional gas mixtures at pressures as low as 5 atm .
	manualset3
252412	2	425700	7	NULL	NULL	0	NULL	CO ( 2 ) laser	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuous frequency tuning of a transversely excited CO ( 2 ) laser was achieved for the 10-microm R branch with conventional gas mixtures at pressures as low as 5 atm .
	manualset3
252413	3	425700	7	NULL	NULL	0	NULL	10-microm R branch	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuous frequency tuning of a transversely excited CO ( 2 ) laser was achieved for the 10-microm R branch with conventional gas mixtures at pressures as low as 5 atm .
	manualset3
252414	4	425700	7	NULL	NULL	0	NULL	conventional gas mixtures 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuous frequency tuning of a transversely excited CO ( 2 ) laser was achieved for the 10-microm R branch with conventional gas mixtures at pressures as low as 5 atm .
	manualset3
252415	5	425700	7	NULL	NULL	0	NULL	 pressures	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuous frequency tuning of a transversely excited CO ( 2 ) laser was achieved for the 10-microm R branch with conventional gas mixtures at pressures as low as 5 atm .
	manualset3
252416	6	425700	7	NULL	NULL	0	NULL	5 atm 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuous frequency tuning of a transversely excited CO ( 2 ) laser was achieved for the 10-microm R branch with conventional gas mixtures at pressures as low as 5 atm .
	manualset3
252417	1	425701	7	NULL	NULL	0	NULL	Continuous glucose monitoring	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuous glucose monitoring during pregnancy in women with polycystic ovary syndrome .
	manualset3
252418	2	425701	7	NULL	NULL	0	NULL	pregnancy	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuous glucose monitoring during pregnancy in women with polycystic ovary syndrome .
	manualset3
252419	3	425701	7	NULL	NULL	0	NULL	 women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuous glucose monitoring during pregnancy in women with polycystic ovary syndrome .
	manualset3
252420	4	425701	7	NULL	NULL	0	NULL	polycystic ovary syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuous glucose monitoring during pregnancy in women with polycystic ovary syndrome .
	manualset3
252421	1	425702	7	NULL	NULL	0	NULL	Continuous infusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuous infusion of the conjunctival sac with chloramphenicol in preoperative cataract patients .
	manualset3
252422	2	425702	7	NULL	NULL	0	NULL	 conjunctival sac	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuous infusion of the conjunctival sac with chloramphenicol in preoperative cataract patients .
	manualset3
252423	3	425702	7	NULL	NULL	0	NULL	chloramphenicol 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuous infusion of the conjunctival sac with chloramphenicol in preoperative cataract patients .
	manualset3
252424	4	425702	7	NULL	NULL	0	NULL	preoperative cataract patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Continuous infusion of the conjunctival sac with chloramphenicol in preoperative cataract patients .
	manualset3
252425	1	425703	7	NULL	NULL	NULL	NULL	Contouring 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Contouring of the cranial vault , especially of the forehead , still is a rarely performed surgical procedure for gender reassignment .
	manualset3
252426	2	425703	7	NULL	NULL	0	NULL	cranial vault	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Contouring of the cranial vault , especially of the forehead , still is a rarely performed surgical procedure for gender reassignment .
	manualset3
252427	3	425703	7	NULL	NULL	0	NULL	forehead	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Contouring of the cranial vault , especially of the forehead , still is a rarely performed surgical procedure for gender reassignment .
	manualset3
252428	4	425703	7	NULL	NULL	0	NULL	surgical procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Contouring of the cranial vault , especially of the forehead , still is a rarely performed surgical procedure for gender reassignment .
	manualset3
252429	5	425703	7	NULL	NULL	0	NULL	gender reassignment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Contouring of the cranial vault , especially of the forehead , still is a rarely performed surgical procedure for gender reassignment .
	manualset3
252430	1	425704	7	NULL	NULL	0	NULL	Contraceptive vaccines	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Contraceptive vaccines for the humane control of community cat populations .
	manualset3
252431	2	425704	7	NULL	NULL	0	NULL	humane control 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Contraceptive vaccines for the humane control of community cat populations .
	manualset3
252432	3	425704	7	NULL	NULL	0	NULL	community cat populations	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Contraceptive vaccines for the humane control of community cat populations .
	manualset3
252433	1	425705	7	NULL	NULL	0	NULL	Contractile response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractile response after ) 48 h to an increase in extracellular calcium concentration ( 1.8 to 2.5 mM ; Fdev increased 43.5 % , n = 2 ) or to 1 microM isoproterenol ( Fdev increased 138.6 % and RT50 decreased 34.9 % , n = 2 ) was similar to those observed in freshly dissected preparations .
	manualset3
252434	2	425705	7	NULL	NULL	0	NULL	48 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractile response after ) 48 h to an increase in extracellular calcium concentration ( 1.8 to 2.5 mM ; Fdev increased 43.5 % , n = 2 ) or to 1 microM isoproterenol ( Fdev increased 138.6 % and RT50 decreased 34.9 % , n = 2 ) was similar to those observed in freshly dissected preparations .
	manualset3
252435	3	425705	7	NULL	NULL	NULL	NULL	increase	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Contractile response after ) 48 h to an increase in extracellular calcium concentration ( 1.8 to 2.5 mM ; Fdev increased 43.5 % , n = 2 ) or to 1 microM isoproterenol ( Fdev increased 138.6 % and RT50 decreased 34.9 % , n = 2 ) was similar to those observed in freshly dissected preparations .
	manualset3
252436	4	425705	7	NULL	NULL	0	NULL	extracellular calcium concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractile response after ) 48 h to an increase in extracellular calcium concentration ( 1.8 to 2.5 mM ; Fdev increased 43.5 % , n = 2 ) or to 1 microM isoproterenol ( Fdev increased 138.6 % and RT50 decreased 34.9 % , n = 2 ) was similar to those observed in freshly dissected preparations .
	manualset3
252437	5	425705	7	NULL	NULL	0	NULL	1.8	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractile response after ) 48 h to an increase in extracellular calcium concentration ( 1.8 to 2.5 mM ; Fdev increased 43.5 % , n = 2 ) or to 1 microM isoproterenol ( Fdev increased 138.6 % and RT50 decreased 34.9 % , n = 2 ) was similar to those observed in freshly dissected preparations .
	manualset3
252438	6	425705	7	NULL	NULL	0	NULL	2.5 mM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractile response after ) 48 h to an increase in extracellular calcium concentration ( 1.8 to 2.5 mM ; Fdev increased 43.5 % , n = 2 ) or to 1 microM isoproterenol ( Fdev increased 138.6 % and RT50 decreased 34.9 % , n = 2 ) was similar to those observed in freshly dissected preparations .
	manualset3
252439	7	425705	7	NULL	NULL	0	NULL	Fdev	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractile response after ) 48 h to an increase in extracellular calcium concentration ( 1.8 to 2.5 mM ; Fdev increased 43.5 % , n = 2 ) or to 1 microM isoproterenol ( Fdev increased 138.6 % and RT50 decreased 34.9 % , n = 2 ) was similar to those observed in freshly dissected preparations .
	manualset3
252440	8	425705	7	NULL	NULL	0	NULL	 43.5 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractile response after ) 48 h to an increase in extracellular calcium concentration ( 1.8 to 2.5 mM ; Fdev increased 43.5 % , n = 2 ) or to 1 microM isoproterenol ( Fdev increased 138.6 % and RT50 decreased 34.9 % , n = 2 ) was similar to those observed in freshly dissected preparations .
	manualset3
252441	9	425705	7	NULL	NULL	0	NULL	n = 2	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractile response after ) 48 h to an increase in extracellular calcium concentration ( 1.8 to 2.5 mM ; Fdev increased 43.5 % , n = 2 ) or to 1 microM isoproterenol ( Fdev increased 138.6 % and RT50 decreased 34.9 % , n = 2 ) was similar to those observed in freshly dissected preparations .
	manualset3
252442	10	425705	7	NULL	NULL	0	NULL	1 microM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractile response after ) 48 h to an increase in extracellular calcium concentration ( 1.8 to 2.5 mM ; Fdev increased 43.5 % , n = 2 ) or to 1 microM isoproterenol ( Fdev increased 138.6 % and RT50 decreased 34.9 % , n = 2 ) was similar to those observed in freshly dissected preparations .
	manualset3
252443	11	425705	7	NULL	NULL	0	NULL	isoproterenol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractile response after ) 48 h to an increase in extracellular calcium concentration ( 1.8 to 2.5 mM ; Fdev increased 43.5 % , n = 2 ) or to 1 microM isoproterenol ( Fdev increased 138.6 % and RT50 decreased 34.9 % , n = 2 ) was similar to those observed in freshly dissected preparations .
	manualset3
252444	12	425705	7	NULL	NULL	0	NULL	 Fdev	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractile response after ) 48 h to an increase in extracellular calcium concentration ( 1.8 to 2.5 mM ; Fdev increased 43.5 % , n = 2 ) or to 1 microM isoproterenol ( Fdev increased 138.6 % and RT50 decreased 34.9 % , n = 2 ) was similar to those observed in freshly dissected preparations .
	manualset3
252445	13	425705	7	NULL	NULL	0	NULL	138.6 % 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractile response after ) 48 h to an increase in extracellular calcium concentration ( 1.8 to 2.5 mM ; Fdev increased 43.5 % , n = 2 ) or to 1 microM isoproterenol ( Fdev increased 138.6 % and RT50 decreased 34.9 % , n = 2 ) was similar to those observed in freshly dissected preparations .
	manualset3
252446	14	425705	7	NULL	NULL	0	NULL	RT50	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractile response after ) 48 h to an increase in extracellular calcium concentration ( 1.8 to 2.5 mM ; Fdev increased 43.5 % , n = 2 ) or to 1 microM isoproterenol ( Fdev increased 138.6 % and RT50 decreased 34.9 % , n = 2 ) was similar to those observed in freshly dissected preparations .
	manualset3
252447	15	425705	7	NULL	NULL	0	NULL	34.9 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractile response after ) 48 h to an increase in extracellular calcium concentration ( 1.8 to 2.5 mM ; Fdev increased 43.5 % , n = 2 ) or to 1 microM isoproterenol ( Fdev increased 138.6 % and RT50 decreased 34.9 % , n = 2 ) was similar to those observed in freshly dissected preparations .
	manualset3
252448	16	425705	7	NULL	NULL	0	NULL	 n = 2	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractile response after ) 48 h to an increase in extracellular calcium concentration ( 1.8 to 2.5 mM ; Fdev increased 43.5 % , n = 2 ) or to 1 microM isoproterenol ( Fdev increased 138.6 % and RT50 decreased 34.9 % , n = 2 ) was similar to those observed in freshly dissected preparations .
	manualset3
252449	17	425705	7	NULL	NULL	0	NULL	freshly dissected preparations	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractile response after ) 48 h to an increase in extracellular calcium concentration ( 1.8 to 2.5 mM ; Fdev increased 43.5 % , n = 2 ) or to 1 microM isoproterenol ( Fdev increased 138.6 % and RT50 decreased 34.9 % , n = 2 ) was similar to those observed in freshly dissected preparations .
	manualset3
252450	1	425706	7	NULL	NULL	0	NULL	Contraction 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contraction of the vastus lateralis , gastrocnemius lateralis , and soleus muscles were determined by the myo-electric activity ( electromyogram , EMG ) by means of surface electrodes .
	manualset3
252451	2	425706	7	NULL	NULL	0	NULL	 vastus lateralis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Contraction of the vastus lateralis , gastrocnemius lateralis , and soleus muscles were determined by the myo-electric activity ( electromyogram , EMG ) by means of surface electrodes .
	manualset3
252452	3	425706	7	NULL	NULL	0	NULL	gastrocnemius lateralis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Contraction of the vastus lateralis , gastrocnemius lateralis , and soleus muscles were determined by the myo-electric activity ( electromyogram , EMG ) by means of surface electrodes .
	manualset3
252453	4	425706	7	NULL	NULL	0	NULL	soleus muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Contraction of the vastus lateralis , gastrocnemius lateralis , and soleus muscles were determined by the myo-electric activity ( electromyogram , EMG ) by means of surface electrodes .
	manualset3
252454	5	425706	7	NULL	NULL	0	NULL	myo-electric activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contraction of the vastus lateralis , gastrocnemius lateralis , and soleus muscles were determined by the myo-electric activity ( electromyogram , EMG ) by means of surface electrodes .
	manualset3
252455	6	425706	7	NULL	NULL	0	NULL	 electromyogram	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Contraction of the vastus lateralis , gastrocnemius lateralis , and soleus muscles were determined by the myo-electric activity ( electromyogram , EMG ) by means of surface electrodes .
	manualset3
252456	7	425706	7	NULL	NULL	0	NULL	EMG	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Contraction of the vastus lateralis , gastrocnemius lateralis , and soleus muscles were determined by the myo-electric activity ( electromyogram , EMG ) by means of surface electrodes .
	manualset3
252457	8	425706	7	NULL	NULL	0	NULL	surface electrodes	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Contraction of the vastus lateralis , gastrocnemius lateralis , and soleus muscles were determined by the myo-electric activity ( electromyogram , EMG ) by means of surface electrodes .
	manualset3
252458	1	425707	7	NULL	NULL	0	NULL	Contractions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractions of the vagally innervated guinea pig tracheal tube preparation were induced by 1 ) stimulation of the preganglionic cervical vagus nerve ( PGS ) , 2 ) activation of postganglionic intrinsic nerves by use of transmural stimulation ( TMS ) in the presence of hexamethonium , and 3 ) exogenous application of spasmogens , acetylcholine ( ACh ) and histamine .
	manualset3
252459	2	425707	7	NULL	NULL	0	NULL	vagally innervated guinea pig tracheal tube preparation	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractions of the vagally innervated guinea pig tracheal tube preparation were induced by 1 ) stimulation of the preganglionic cervical vagus nerve ( PGS ) , 2 ) activation of postganglionic intrinsic nerves by use of transmural stimulation ( TMS ) in the presence of hexamethonium , and 3 ) exogenous application of spasmogens , acetylcholine ( ACh ) and histamine .
	manualset3
252460	3	425707	7	NULL	NULL	0	NULL	 stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractions of the vagally innervated guinea pig tracheal tube preparation were induced by 1 ) stimulation of the preganglionic cervical vagus nerve ( PGS ) , 2 ) activation of postganglionic intrinsic nerves by use of transmural stimulation ( TMS ) in the presence of hexamethonium , and 3 ) exogenous application of spasmogens , acetylcholine ( ACh ) and histamine .
	manualset3
252461	4	425707	7	NULL	NULL	0	NULL	 preganglionic cervical vagus nerve ( PGS )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractions of the vagally innervated guinea pig tracheal tube preparation were induced by 1 ) stimulation of the preganglionic cervical vagus nerve ( PGS ) , 2 ) activation of postganglionic intrinsic nerves by use of transmural stimulation ( TMS ) in the presence of hexamethonium , and 3 ) exogenous application of spasmogens , acetylcholine ( ACh ) and histamine .
	manualset3
252462	5	425707	7	NULL	NULL	0	NULL	 activation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractions of the vagally innervated guinea pig tracheal tube preparation were induced by 1 ) stimulation of the preganglionic cervical vagus nerve ( PGS ) , 2 ) activation of postganglionic intrinsic nerves by use of transmural stimulation ( TMS ) in the presence of hexamethonium , and 3 ) exogenous application of spasmogens , acetylcholine ( ACh ) and histamine .
	manualset3
252463	6	425707	7	NULL	NULL	0	NULL	postganglionic intrinsic nerves	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractions of the vagally innervated guinea pig tracheal tube preparation were induced by 1 ) stimulation of the preganglionic cervical vagus nerve ( PGS ) , 2 ) activation of postganglionic intrinsic nerves by use of transmural stimulation ( TMS ) in the presence of hexamethonium , and 3 ) exogenous application of spasmogens , acetylcholine ( ACh ) and histamine .
	manualset3
252464	7	425707	7	NULL	NULL	0	NULL	 use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractions of the vagally innervated guinea pig tracheal tube preparation were induced by 1 ) stimulation of the preganglionic cervical vagus nerve ( PGS ) , 2 ) activation of postganglionic intrinsic nerves by use of transmural stimulation ( TMS ) in the presence of hexamethonium , and 3 ) exogenous application of spasmogens , acetylcholine ( ACh ) and histamine .
	manualset3
252465	8	425707	7	NULL	NULL	0	NULL	transmural stimulation ( TMS )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractions of the vagally innervated guinea pig tracheal tube preparation were induced by 1 ) stimulation of the preganglionic cervical vagus nerve ( PGS ) , 2 ) activation of postganglionic intrinsic nerves by use of transmural stimulation ( TMS ) in the presence of hexamethonium , and 3 ) exogenous application of spasmogens , acetylcholine ( ACh ) and histamine .
	manualset3
252466	9	425707	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractions of the vagally innervated guinea pig tracheal tube preparation were induced by 1 ) stimulation of the preganglionic cervical vagus nerve ( PGS ) , 2 ) activation of postganglionic intrinsic nerves by use of transmural stimulation ( TMS ) in the presence of hexamethonium , and 3 ) exogenous application of spasmogens , acetylcholine ( ACh ) and histamine .
	manualset3
252467	10	425707	7	NULL	NULL	0	NULL	hexamethonium 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractions of the vagally innervated guinea pig tracheal tube preparation were induced by 1 ) stimulation of the preganglionic cervical vagus nerve ( PGS ) , 2 ) activation of postganglionic intrinsic nerves by use of transmural stimulation ( TMS ) in the presence of hexamethonium , and 3 ) exogenous application of spasmogens , acetylcholine ( ACh ) and histamine .
	manualset3
252468	11	425707	7	NULL	NULL	0	NULL	exogenous application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractions of the vagally innervated guinea pig tracheal tube preparation were induced by 1 ) stimulation of the preganglionic cervical vagus nerve ( PGS ) , 2 ) activation of postganglionic intrinsic nerves by use of transmural stimulation ( TMS ) in the presence of hexamethonium , and 3 ) exogenous application of spasmogens , acetylcholine ( ACh ) and histamine .
	manualset3
252469	12	425707	7	NULL	NULL	0	NULL	spasmogens	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractions of the vagally innervated guinea pig tracheal tube preparation were induced by 1 ) stimulation of the preganglionic cervical vagus nerve ( PGS ) , 2 ) activation of postganglionic intrinsic nerves by use of transmural stimulation ( TMS ) in the presence of hexamethonium , and 3 ) exogenous application of spasmogens , acetylcholine ( ACh ) and histamine .
	manualset3
252470	13	425707	7	NULL	NULL	0	NULL	acetylcholine ( ACh )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractions of the vagally innervated guinea pig tracheal tube preparation were induced by 1 ) stimulation of the preganglionic cervical vagus nerve ( PGS ) , 2 ) activation of postganglionic intrinsic nerves by use of transmural stimulation ( TMS ) in the presence of hexamethonium , and 3 ) exogenous application of spasmogens , acetylcholine ( ACh ) and histamine .
	manualset3
252471	14	425707	7	NULL	NULL	0	NULL	histamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractions of the vagally innervated guinea pig tracheal tube preparation were induced by 1 ) stimulation of the preganglionic cervical vagus nerve ( PGS ) , 2 ) activation of postganglionic intrinsic nerves by use of transmural stimulation ( TMS ) in the presence of hexamethonium , and 3 ) exogenous application of spasmogens , acetylcholine ( ACh ) and histamine .
	manualset3
252472	1	425708	7	NULL	NULL	0	NULL	Contractures	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractures including pseudoainhum were also observed in some children .
	manualset3
252473	2	425708	7	NULL	NULL	0	NULL	pseudoainhum 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractures including pseudoainhum were also observed in some children .
	manualset3
252474	3	425708	7	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Contractures including pseudoainhum were also observed in some children .
	manualset3
252475	1	425709	7	NULL	NULL	0	NULL	Localized cortical atrophy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Localized cortical atrophy in primary lateral sclerosis ) .
	manualset3
252476	2	425709	7	NULL	NULL	0	NULL	primary lateral sclerosis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Localized cortical atrophy in primary lateral sclerosis ) .
	manualset3
252477	1	425710	7	NULL	NULL	0	NULL	Contralateral locus fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Contralateral locus fibers reach the CN by crossing in the pontine central gray at the rostral border of the fourth ventricle and by decussating with the fibers of the mesencephalic trigeminal nucleus ventral to the medial longitudinal fasciculus .
	manualset3
252479	2	425710	7	NULL	NULL	NULL	NULL	CN	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Contralateral locus fibers reach the CN by crossing in the pontine central gray at the rostral border of the fourth ventricle and by decussating with the fibers of the mesencephalic trigeminal nucleus ventral to the medial longitudinal fasciculus .
	manualset3
252480	3	425710	7	NULL	NULL	0	NULL	pontine central gray	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Contralateral locus fibers reach the CN by crossing in the pontine central gray at the rostral border of the fourth ventricle and by decussating with the fibers of the mesencephalic trigeminal nucleus ventral to the medial longitudinal fasciculus .
	manualset3
252481	4	425710	7	NULL	NULL	0	NULL	 rostral border	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Contralateral locus fibers reach the CN by crossing in the pontine central gray at the rostral border of the fourth ventricle and by decussating with the fibers of the mesencephalic trigeminal nucleus ventral to the medial longitudinal fasciculus .
	manualset3
252482	5	425710	7	NULL	NULL	0	NULL	 fourth ventricle 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Contralateral locus fibers reach the CN by crossing in the pontine central gray at the rostral border of the fourth ventricle and by decussating with the fibers of the mesencephalic trigeminal nucleus ventral to the medial longitudinal fasciculus .
	manualset3
252483	6	425710	7	NULL	NULL	0	NULL	fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Contralateral locus fibers reach the CN by crossing in the pontine central gray at the rostral border of the fourth ventricle and by decussating with the fibers of the mesencephalic trigeminal nucleus ventral to the medial longitudinal fasciculus .
	manualset3
252484	7	425710	7	NULL	NULL	0	NULL	mesencephalic trigeminal nucleus ventral	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Contralateral locus fibers reach the CN by crossing in the pontine central gray at the rostral border of the fourth ventricle and by decussating with the fibers of the mesencephalic trigeminal nucleus ventral to the medial longitudinal fasciculus .
	manualset3
252485	8	425710	7	NULL	NULL	0	NULL	medial longitudinal fasciculus 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Contralateral locus fibers reach the CN by crossing in the pontine central gray at the rostral border of the fourth ventricle and by decussating with the fibers of the mesencephalic trigeminal nucleus ventral to the medial longitudinal fasciculus .
	manualset3
252486	1	425711	7	NULL	NULL	0	NULL	 expectations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to expectations , elevations of endogenous ET-1 levels in transgenic mice are not associated with increases in arterial blood pressure or with vasospasm , although these effects can be observed after i.v. ET-1 administration .
	manualset3
252487	2	425711	7	NULL	NULL	0	NULL	elevations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to expectations , elevations of endogenous ET-1 levels in transgenic mice are not associated with increases in arterial blood pressure or with vasospasm , although these effects can be observed after i.v. ET-1 administration .
	manualset3
252488	3	425711	7	NULL	NULL	0	NULL	endogenous ET-1 levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to expectations , elevations of endogenous ET-1 levels in transgenic mice are not associated with increases in arterial blood pressure or with vasospasm , although these effects can be observed after i.v. ET-1 administration .
	manualset3
252489	4	425711	7	NULL	NULL	0	NULL	transgenic mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to expectations , elevations of endogenous ET-1 levels in transgenic mice are not associated with increases in arterial blood pressure or with vasospasm , although these effects can be observed after i.v. ET-1 administration .
	manualset3
252490	5	425711	7	NULL	NULL	NULL	NULL	arterial blood pressure	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Contrary to expectations , elevations of endogenous ET-1 levels in transgenic mice are not associated with increases in arterial blood pressure or with vasospasm , although these effects can be observed after i.v. ET-1 administration .
	manualset3
252491	6	425711	7	NULL	NULL	0	NULL	 vasospasm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to expectations , elevations of endogenous ET-1 levels in transgenic mice are not associated with increases in arterial blood pressure or with vasospasm , although these effects can be observed after i.v. ET-1 administration .
	manualset3
252492	7	425711	7	NULL	NULL	0	NULL	effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to expectations , elevations of endogenous ET-1 levels in transgenic mice are not associated with increases in arterial blood pressure or with vasospasm , although these effects can be observed after i.v. ET-1 administration .
	manualset3
252493	8	425711	7	NULL	NULL	0	NULL	 i.v. ET-1 administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to expectations , elevations of endogenous ET-1 levels in transgenic mice are not associated with increases in arterial blood pressure or with vasospasm , although these effects can be observed after i.v. ET-1 administration .
	manualset3
252494	1	425712	7	NULL	NULL	0	NULL	expectations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to expectations for non-precocial chicks , this pattern of corticosterone responses to handling indicates that grey-faced petrel chicks are able to perceive and respond to potential stressors from hatching , a response previously only demonstrated for precocial birds .
	manualset3
252495	2	425712	7	NULL	NULL	0	NULL	 non-precocial chicks	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to expectations for non-precocial chicks , this pattern of corticosterone responses to handling indicates that grey-faced petrel chicks are able to perceive and respond to potential stressors from hatching , a response previously only demonstrated for precocial birds .
	manualset3
252496	3	425712	7	NULL	NULL	0	NULL	pattern	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to expectations for non-precocial chicks , this pattern of corticosterone responses to handling indicates that grey-faced petrel chicks are able to perceive and respond to potential stressors from hatching , a response previously only demonstrated for precocial birds .
	manualset3
252497	4	425712	7	NULL	NULL	0	NULL	corticosterone	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to expectations for non-precocial chicks , this pattern of corticosterone responses to handling indicates that grey-faced petrel chicks are able to perceive and respond to potential stressors from hatching , a response previously only demonstrated for precocial birds .
	manualset3
252498	5	425712	7	NULL	NULL	0	NULL	handling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to expectations for non-precocial chicks , this pattern of corticosterone responses to handling indicates that grey-faced petrel chicks are able to perceive and respond to potential stressors from hatching , a response previously only demonstrated for precocial birds .
	manualset3
252499	6	425712	7	NULL	NULL	0	NULL	 grey-faced petrel chicks	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to expectations for non-precocial chicks , this pattern of corticosterone responses to handling indicates that grey-faced petrel chicks are able to perceive and respond to potential stressors from hatching , a response previously only demonstrated for precocial birds .
	manualset3
252500	7	425712	7	NULL	NULL	0	NULL	potential stressors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to expectations for non-precocial chicks , this pattern of corticosterone responses to handling indicates that grey-faced petrel chicks are able to perceive and respond to potential stressors from hatching , a response previously only demonstrated for precocial birds .
	manualset3
252501	8	425712	7	NULL	NULL	0	NULL	hatching	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to expectations for non-precocial chicks , this pattern of corticosterone responses to handling indicates that grey-faced petrel chicks are able to perceive and respond to potential stressors from hatching , a response previously only demonstrated for precocial birds .
	manualset3
252502	9	425712	7	NULL	NULL	0	NULL	response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to expectations for non-precocial chicks , this pattern of corticosterone responses to handling indicates that grey-faced petrel chicks are able to perceive and respond to potential stressors from hatching , a response previously only demonstrated for precocial birds .
	manualset3
252503	10	425712	7	NULL	NULL	0	NULL	precocial birds	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to expectations for non-precocial chicks , this pattern of corticosterone responses to handling indicates that grey-faced petrel chicks are able to perceive and respond to potential stressors from hatching , a response previously only demonstrated for precocial birds .
	manualset3
252504	1	425713	7	NULL	NULL	0	NULL	infrequent injections	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to infrequent injections of small amounts of calcium which evoked smooth transient responses , these fluctuating chloride currents are due to overloading of intracellular calcium stores which then release calcium repeatedly .
	manualset3
252505	2	425713	7	NULL	NULL	0	NULL	small amounts 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to infrequent injections of small amounts of calcium which evoked smooth transient responses , these fluctuating chloride currents are due to overloading of intracellular calcium stores which then release calcium repeatedly .
	manualset3
252506	3	425713	7	NULL	NULL	0	NULL	calcium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to infrequent injections of small amounts of calcium which evoked smooth transient responses , these fluctuating chloride currents are due to overloading of intracellular calcium stores which then release calcium repeatedly .
	manualset3
252507	4	425713	7	NULL	NULL	0	NULL	smooth transient responses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to infrequent injections of small amounts of calcium which evoked smooth transient responses , these fluctuating chloride currents are due to overloading of intracellular calcium stores which then release calcium repeatedly .
	manualset3
252508	5	425713	7	NULL	NULL	0	NULL	chloride currents	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to infrequent injections of small amounts of calcium which evoked smooth transient responses , these fluctuating chloride currents are due to overloading of intracellular calcium stores which then release calcium repeatedly .
	manualset3
252509	6	425713	7	NULL	NULL	0	NULL	overloading	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to infrequent injections of small amounts of calcium which evoked smooth transient responses , these fluctuating chloride currents are due to overloading of intracellular calcium stores which then release calcium repeatedly .
	manualset3
252510	7	425713	7	NULL	NULL	0	NULL	intracellular calcium stores	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to infrequent injections of small amounts of calcium which evoked smooth transient responses , these fluctuating chloride currents are due to overloading of intracellular calcium stores which then release calcium repeatedly .
	manualset3
252511	8	425713	7	NULL	NULL	0	NULL	calcium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to infrequent injections of small amounts of calcium which evoked smooth transient responses , these fluctuating chloride currents are due to overloading of intracellular calcium stores which then release calcium repeatedly .
	manualset3
252512	1	425714	7	NULL	NULL	0	NULL	prediction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to prediction , fathers who reported less seeking support and adaptive-focused coping showed the most improvement in their children 's behavior .
	manualset3
252513	2	425714	7	NULL	NULL	0	NULL	 fathers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to prediction , fathers who reported less seeking support and adaptive-focused coping showed the most improvement in their children 's behavior .
	manualset3
252514	3	425714	7	NULL	NULL	0	NULL	 support 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to prediction , fathers who reported less seeking support and adaptive-focused coping showed the most improvement in their children 's behavior .
	manualset3
252515	4	425714	7	NULL	NULL	0	NULL	adaptive-focused coping	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to prediction , fathers who reported less seeking support and adaptive-focused coping showed the most improvement in their children 's behavior .
	manualset3
252516	5	425714	7	NULL	NULL	0	NULL	 improvement 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to prediction , fathers who reported less seeking support and adaptive-focused coping showed the most improvement in their children 's behavior .
	manualset3
252517	6	425714	7	NULL	NULL	0	NULL	children 's behavior	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to prediction , fathers who reported less seeking support and adaptive-focused coping showed the most improvement in their children 's behavior .
	manualset3
252518	1	425715	7	NULL	NULL	0	NULL	 prediction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to prediction , no reliable picture advantages emerged .
	manualset3
252519	2	425715	7	NULL	NULL	0	NULL	picture	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to prediction , no reliable picture advantages emerged .
	manualset3
252520	1	425716	7	NULL	NULL	0	NULL	considerations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to previous considerations evidence suggests that astrocytes , glioma cells and tumor endothelial cells may all have pivotal roles in the initiation and prolongation of both local and systemic immune responses to the tumor .
	manualset3
252521	2	425716	7	NULL	NULL	0	NULL	evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to previous considerations evidence suggests that astrocytes , glioma cells and tumor endothelial cells may all have pivotal roles in the initiation and prolongation of both local and systemic immune responses to the tumor .
	manualset3
252522	3	425716	7	NULL	NULL	0	NULL	astrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to previous considerations evidence suggests that astrocytes , glioma cells and tumor endothelial cells may all have pivotal roles in the initiation and prolongation of both local and systemic immune responses to the tumor .
	manualset3
252523	4	425716	7	NULL	NULL	0	NULL	glioma cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to previous considerations evidence suggests that astrocytes , glioma cells and tumor endothelial cells may all have pivotal roles in the initiation and prolongation of both local and systemic immune responses to the tumor .
	manualset3
252524	5	425716	7	NULL	NULL	0	NULL	tumor endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to previous considerations evidence suggests that astrocytes , glioma cells and tumor endothelial cells may all have pivotal roles in the initiation and prolongation of both local and systemic immune responses to the tumor .
	manualset3
252525	6	425716	7	NULL	NULL	0	NULL	pivotal roles	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to previous considerations evidence suggests that astrocytes , glioma cells and tumor endothelial cells may all have pivotal roles in the initiation and prolongation of both local and systemic immune responses to the tumor .
	manualset3
252526	7	425716	7	NULL	NULL	0	NULL	 initiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to previous considerations evidence suggests that astrocytes , glioma cells and tumor endothelial cells may all have pivotal roles in the initiation and prolongation of both local and systemic immune responses to the tumor .
	manualset3
252527	8	425716	7	NULL	NULL	0	NULL	prolongation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to previous considerations evidence suggests that astrocytes , glioma cells and tumor endothelial cells may all have pivotal roles in the initiation and prolongation of both local and systemic immune responses to the tumor .
	manualset3
252528	9	425716	7	NULL	NULL	0	NULL	local immune response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to previous considerations evidence suggests that astrocytes , glioma cells and tumor endothelial cells may all have pivotal roles in the initiation and prolongation of both local and systemic immune responses to the tumor .
	manualset3
252529	10	425716	7	NULL	NULL	0	NULL	systemic immune responses	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to previous considerations evidence suggests that astrocytes , glioma cells and tumor endothelial cells may all have pivotal roles in the initiation and prolongation of both local and systemic immune responses to the tumor .
	manualset3
252530	11	425716	7	NULL	NULL	0	NULL	 tumor	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrary to previous considerations evidence suggests that astrocytes , glioma cells and tumor endothelial cells may all have pivotal roles in the initiation and prolongation of both local and systemic immune responses to the tumor .
	manualset3
252531	1	425717	7	NULL	NULL	0	NULL	Long-term dialysis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Long-term dialysis and its problems : introduction ) .
	manualset3
252532	2	425717	7	NULL	NULL	0	NULL	problems	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Long-term dialysis and its problems : introduction ) .
	manualset3
252533	3	425717	7	NULL	NULL	0	NULL	introduction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Long-term dialysis and its problems : introduction ) .
	manualset3
252534	1	425718	7	NULL	NULL	0	NULL	enhanced CT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrast enhanced CT is the imaging modality of choice for depicting its morphology and extension .
	manualset3
252535	2	425718	7	NULL	NULL	0	NULL	imaging modality	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrast enhanced CT is the imaging modality of choice for depicting its morphology and extension .
	manualset3
252536	3	425718	7	NULL	NULL	0	NULL	morphology	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrast enhanced CT is the imaging modality of choice for depicting its morphology and extension .
	manualset3
252537	4	425718	7	NULL	NULL	0	NULL	extension	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrast enhanced CT is the imaging modality of choice for depicting its morphology and extension .
	manualset3
252538	1	425719	7	NULL	NULL	0	NULL	Contrast enhancement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrast enhancement of the spinal cord in a patient with cervical spondylotic myelopathy .
	manualset3
252539	2	425719	7	NULL	NULL	0	NULL	 spinal cord 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrast enhancement of the spinal cord in a patient with cervical spondylotic myelopathy .
	manualset3
252540	3	425719	7	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrast enhancement of the spinal cord in a patient with cervical spondylotic myelopathy .
	manualset3
252542	4	425719	7	NULL	NULL	0	NULL	cervical spondylotic myelopathy 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Contrast enhancement of the spinal cord in a patient with cervical spondylotic myelopathy .
	manualset3
252543	1	425720	7	NULL	NULL	0	NULL	Contribution 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contribution by breastfeeding was an important exogenous source for regulating plasma OXT before weaning by the presence of OXT in milk and the dam 's mammary glands .
	manualset3
252544	2	425720	7	NULL	NULL	0	NULL	breastfeeding	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contribution by breastfeeding was an important exogenous source for regulating plasma OXT before weaning by the presence of OXT in milk and the dam 's mammary glands .
	manualset3
252545	3	425720	7	NULL	NULL	0	NULL	exogenous source	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contribution by breastfeeding was an important exogenous source for regulating plasma OXT before weaning by the presence of OXT in milk and the dam 's mammary glands .
	manualset3
252546	4	425720	7	NULL	NULL	0	NULL	plasma OXT	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Contribution by breastfeeding was an important exogenous source for regulating plasma OXT before weaning by the presence of OXT in milk and the dam 's mammary glands .
	manualset3
252547	5	425720	7	NULL	NULL	0	NULL	 weaning	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contribution by breastfeeding was an important exogenous source for regulating plasma OXT before weaning by the presence of OXT in milk and the dam 's mammary glands .
	manualset3
252548	6	425720	7	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contribution by breastfeeding was an important exogenous source for regulating plasma OXT before weaning by the presence of OXT in milk and the dam 's mammary glands .
	manualset3
252549	7	425720	7	NULL	NULL	0	NULL	OXT	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contribution by breastfeeding was an important exogenous source for regulating plasma OXT before weaning by the presence of OXT in milk and the dam 's mammary glands .
	manualset3
252550	8	425720	7	NULL	NULL	0	NULL	 milk	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Contribution by breastfeeding was an important exogenous source for regulating plasma OXT before weaning by the presence of OXT in milk and the dam 's mammary glands .
	manualset3
252551	9	425720	7	NULL	NULL	0	NULL	dam 's mammary glands 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Contribution by breastfeeding was an important exogenous source for regulating plasma OXT before weaning by the presence of OXT in milk and the dam 's mammary glands .
	manualset3
252552	1	425721	7	NULL	NULL	0	NULL	Contribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contribution of NMDA receptors to tetanus-induced increase in postsynaptic Ca2 + in visual cortex of young rats .
	manualset3
252553	2	425721	7	NULL	NULL	0	NULL	NMDA receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Contribution of NMDA receptors to tetanus-induced increase in postsynaptic Ca2 + in visual cortex of young rats .
	manualset3
252554	3	425721	7	NULL	NULL	0	NULL	tetanus-induced increase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contribution of NMDA receptors to tetanus-induced increase in postsynaptic Ca2 + in visual cortex of young rats .
	manualset3
252555	4	425721	7	NULL	NULL	0	NULL	postsynaptic Ca2 +	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Contribution of NMDA receptors to tetanus-induced increase in postsynaptic Ca2 + in visual cortex of young rats .
	manualset3
252556	5	425721	7	NULL	NULL	0	NULL	visual cortex 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Contribution of NMDA receptors to tetanus-induced increase in postsynaptic Ca2 + in visual cortex of young rats .
	manualset3
252557	6	425721	7	NULL	NULL	0	NULL	 young rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Contribution of NMDA receptors to tetanus-induced increase in postsynaptic Ca2 + in visual cortex of young rats .
	manualset3
252558	1	425722	7	NULL	NULL	0	NULL	Contribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contribution of carbohydrate antigens sialyl Lewis A and sialyl Lewis X to adhesion of human cancer cells to vascular endothelium .
	manualset3
252559	2	425722	7	NULL	NULL	0	NULL	carbohydrate antigens	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Contribution of carbohydrate antigens sialyl Lewis A and sialyl Lewis X to adhesion of human cancer cells to vascular endothelium .
	manualset3
252560	3	425722	7	NULL	NULL	0	NULL	sialyl Lewis A	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Contribution of carbohydrate antigens sialyl Lewis A and sialyl Lewis X to adhesion of human cancer cells to vascular endothelium .
	manualset3
252561	4	425722	7	NULL	NULL	0	NULL	sialyl Lewis X	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Contribution of carbohydrate antigens sialyl Lewis A and sialyl Lewis X to adhesion of human cancer cells to vascular endothelium .
	manualset3
252562	5	425722	7	NULL	NULL	0	NULL	adhesion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contribution of carbohydrate antigens sialyl Lewis A and sialyl Lewis X to adhesion of human cancer cells to vascular endothelium .
	manualset3
252563	6	425722	7	NULL	NULL	0	NULL	human cancer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Contribution of carbohydrate antigens sialyl Lewis A and sialyl Lewis X to adhesion of human cancer cells to vascular endothelium .
	manualset3
252564	7	425722	7	NULL	NULL	NULL	NULL	vascular endothelium	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Contribution of carbohydrate antigens sialyl Lewis A and sialyl Lewis X to adhesion of human cancer cells to vascular endothelium .
	manualset3
252565	1	425723	7	NULL	NULL	0	NULL	Contribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contribution of the NADH-oxidase ( Nox ) to the aerobic life of Lactobacillus sanfranciscensis DSM20451T .
	manualset3
252566	2	425723	7	NULL	NULL	0	NULL	NADH-oxidase ( Nox )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Contribution of the NADH-oxidase ( Nox ) to the aerobic life of Lactobacillus sanfranciscensis DSM20451T .
	manualset3
252567	3	425723	7	NULL	NULL	0	NULL	aerobic life	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contribution of the NADH-oxidase ( Nox ) to the aerobic life of Lactobacillus sanfranciscensis DSM20451T .
	manualset3
252568	4	425723	7	NULL	NULL	0	NULL	Lactobacillus sanfranciscensis DSM20451T	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Contribution of the NADH-oxidase ( Nox ) to the aerobic life of Lactobacillus sanfranciscensis DSM20451T .
	manualset3
252569	1	425724	7	NULL	NULL	0	NULL	Contribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contribution of thymidylate synthase to gemcitabine therapy for advanced pancreatic cancer .
	manualset3
252570	2	425724	7	NULL	NULL	0	NULL	thymidylate synthase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Contribution of thymidylate synthase to gemcitabine therapy for advanced pancreatic cancer .
	manualset3
252571	3	425724	7	NULL	NULL	0	NULL	gemcitabine therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Contribution of thymidylate synthase to gemcitabine therapy for advanced pancreatic cancer .
	manualset3
252572	4	425724	7	NULL	NULL	0	NULL	advanced pancreatic cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Contribution of thymidylate synthase to gemcitabine therapy for advanced pancreatic cancer .
	manualset3
252573	1	425725	7	NULL	NULL	0	NULL	Contributions	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Contributions of quisqualate and NMDA receptors to the induction and expression of LTP .
	manualset3
252574	2	425725	7	NULL	NULL	0	NULL	quisqualate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Contributions of quisqualate and NMDA receptors to the induction and expression of LTP .
	manualset3
252575	3	425725	7	NULL	NULL	0	NULL	NMDA receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Contributions of quisqualate and NMDA receptors to the induction and expression of LTP .
	manualset3
252576	4	425725	7	NULL	NULL	0	NULL	induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contributions of quisqualate and NMDA receptors to the induction and expression of LTP .
	manualset3
252577	5	425725	7	NULL	NULL	0	NULL	 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contributions of quisqualate and NMDA receptors to the induction and expression of LTP .
	manualset3
252578	6	425725	7	NULL	NULL	0	NULL	LTP	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Contributions of quisqualate and NMDA receptors to the induction and expression of LTP .
	manualset3
252579	1	425726	7	NULL	NULL	0	NULL	Long-term follow-up	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	( Long-term follow-up of 52 endoluminal irradiated patients with central lung tumors ) .
	manualset3
252580	2	425726	7	NULL	NULL	0	NULL	52 endoluminal irradiated patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Long-term follow-up of 52 endoluminal irradiated patients with central lung tumors ) .
	manualset3
252581	3	425726	7	NULL	NULL	0	NULL	central lung tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Long-term follow-up of 52 endoluminal irradiated patients with central lung tumors ) .
	manualset3
252582	1	425727	7	NULL	NULL	0	NULL	Control 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Control : Chemical control and breeding programs for disease resistance .
	manualset3
252583	2	425727	7	NULL	NULL	0	NULL	Chemical control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Control : Chemical control and breeding programs for disease resistance .
	manualset3
252584	3	425727	7	NULL	NULL	0	NULL	breeding programs	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Control : Chemical control and breeding programs for disease resistance .
	manualset3
252585	4	425727	7	NULL	NULL	0	NULL	disease resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Control : Chemical control and breeding programs for disease resistance .
	manualset3
252586	1	425728	7	NULL	NULL	0	NULL	Control DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Control DNA was extracted from urine or peripheral blood samples from the healthy women .
	manualset3
252587	2	425728	7	NULL	NULL	0	NULL	urine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Control DNA was extracted from urine or peripheral blood samples from the healthy women .
	manualset3
252588	3	425728	7	NULL	NULL	0	NULL	peripheral blood samples	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Control DNA was extracted from urine or peripheral blood samples from the healthy women .
	manualset3
252589	4	425728	7	NULL	NULL	0	NULL	 healthy women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Control DNA was extracted from urine or peripheral blood samples from the healthy women .
	manualset3
252590	1	425729	7	NULL	NULL	0	NULL	Control experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Control experiments with appropriate model compounds indicate that the local excitation of the oxazine component results first in intersystem crossing and then energy transfer to the BODIPY component .
	manualset3
252591	2	425729	7	NULL	NULL	0	NULL	appropriate model compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Control experiments with appropriate model compounds indicate that the local excitation of the oxazine component results first in intersystem crossing and then energy transfer to the BODIPY component .
	manualset3
252592	3	425729	7	NULL	NULL	0	NULL	local excitation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Control experiments with appropriate model compounds indicate that the local excitation of the oxazine component results first in intersystem crossing and then energy transfer to the BODIPY component .
	manualset3
252593	4	425729	7	NULL	NULL	0	NULL	oxazine component	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Control experiments with appropriate model compounds indicate that the local excitation of the oxazine component results first in intersystem crossing and then energy transfer to the BODIPY component .
	manualset3
252594	5	425729	7	NULL	NULL	0	NULL	intersystem crossing	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Control experiments with appropriate model compounds indicate that the local excitation of the oxazine component results first in intersystem crossing and then energy transfer to the BODIPY component .
	manualset3
252595	6	425729	7	NULL	NULL	0	NULL	energy transfer	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Control experiments with appropriate model compounds indicate that the local excitation of the oxazine component results first in intersystem crossing and then energy transfer to the BODIPY component .
	manualset3
252596	7	425729	7	NULL	NULL	0	NULL	BODIPY component	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Control experiments with appropriate model compounds indicate that the local excitation of the oxazine component results first in intersystem crossing and then energy transfer to the BODIPY component .
	manualset3
252597	1	425730	7	NULL	NULL	0	NULL	Control human DNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Control human and Chinese hamster DNAs displayed a distinct Eco R1 restriction fragment pattern when hybridized with the human Cx50 DNA probe .
	manualset3
252598	2	425730	7	NULL	NULL	0	NULL	Chinese hamster DNAs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Control human and Chinese hamster DNAs displayed a distinct Eco R1 restriction fragment pattern when hybridized with the human Cx50 DNA probe .
	manualset3
252599	3	425730	7	NULL	NULL	0	NULL	Eco R1 restriction fragment pattern	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Control human and Chinese hamster DNAs displayed a distinct Eco R1 restriction fragment pattern when hybridized with the human Cx50 DNA probe .
	manualset3
252600	4	425730	7	NULL	NULL	0	NULL	human Cx50 DNA probe	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Control human and Chinese hamster DNAs displayed a distinct Eco R1 restriction fragment pattern when hybridized with the human Cx50 DNA probe .
	manualset3
252922	1	425731	7	NULL	NULL	0	NULL	Control 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of arbovirus infections by a coordinated response : West Nile Virus in England and Wales .
	manualset3
252923	2	425731	7	NULL	NULL	0	NULL	coordinated response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of arbovirus infections by a coordinated response : West Nile Virus in England and Wales .
	manualset3
252924	3	425731	7	NULL	NULL	0	NULL	West Nile Virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of arbovirus infections by a coordinated response : West Nile Virus in England and Wales .
	manualset3
252925	4	425731	7	NULL	NULL	0	NULL	England 	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of arbovirus infections by a coordinated response : West Nile Virus in England and Wales .
	manualset3
252926	5	425731	7	NULL	NULL	0	NULL	Wales	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of arbovirus infections by a coordinated response : West Nile Virus in England and Wales .
	manualset3
252927	6	425731	7	NULL	NULL	0	NULL	arbovirus infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of arbovirus infections by a coordinated response : West Nile Virus in England and Wales .
	manualset3
252928	1	425732	7	NULL	NULL	0	NULL	Control 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of final organ size by Mediator complex subunit 25 in Arabidopsis thaliana .
	manualset3
252929	2	425732	7	NULL	NULL	0	NULL	final organ size	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of final organ size by Mediator complex subunit 25 in Arabidopsis thaliana .
	manualset3
252930	3	425732	7	NULL	NULL	0	NULL	Mediator complex subunit 25	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of final organ size by Mediator complex subunit 25 in Arabidopsis thaliana .
	manualset3
252931	4	425732	7	NULL	NULL	0	NULL	Arabidopsis thaliana	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of final organ size by Mediator complex subunit 25 in Arabidopsis thaliana .
	manualset3
252932	1	425733	7	NULL	NULL	0	NULL	Control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of pain was achieved in 66 percent of cases .
	manualset3
252933	2	425733	7	NULL	NULL	0	NULL	 pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of pain was achieved in 66 percent of cases .
	manualset3
252934	3	425733	7	NULL	NULL	0	NULL	 66 percent	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of pain was achieved in 66 percent of cases .
	manualset3
252935	4	425733	7	NULL	NULL	0	NULL	cases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of pain was achieved in 66 percent of cases .
	manualset3
252936	1	425734	7	NULL	NULL	0	NULL	Long-term surgical results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Long-term surgical results in cancer of the larynx ) .
	manualset3
252937	2	425734	7	NULL	NULL	0	NULL	cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Long-term surgical results in cancer of the larynx ) .
	manualset3
252938	3	425734	7	NULL	NULL	0	NULL	larynx 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Long-term surgical results in cancer of the larynx ) .
	manualset3
252939	1	425735	7	NULL	NULL	0	NULL	Control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of the timing of labeling and mitotic index peaks by different parameters of the LD cycle suggests a mechanism for cell cycle regulation by the environmental lighting schedule .
	manualset3
252940	2	425735	7	NULL	NULL	0	NULL	 timing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of the timing of labeling and mitotic index peaks by different parameters of the LD cycle suggests a mechanism for cell cycle regulation by the environmental lighting schedule .
	manualset3
252941	3	425735	7	NULL	NULL	0	NULL	 labeling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of the timing of labeling and mitotic index peaks by different parameters of the LD cycle suggests a mechanism for cell cycle regulation by the environmental lighting schedule .
	manualset3
252942	4	425735	7	NULL	NULL	0	NULL	mitotic index peaks	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of the timing of labeling and mitotic index peaks by different parameters of the LD cycle suggests a mechanism for cell cycle regulation by the environmental lighting schedule .
	manualset3
252943	5	425735	7	NULL	NULL	0	NULL	different parameters 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of the timing of labeling and mitotic index peaks by different parameters of the LD cycle suggests a mechanism for cell cycle regulation by the environmental lighting schedule .
	manualset3
252944	6	425735	7	NULL	NULL	0	NULL	LD cycle 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of the timing of labeling and mitotic index peaks by different parameters of the LD cycle suggests a mechanism for cell cycle regulation by the environmental lighting schedule .
	manualset3
252945	7	425735	7	NULL	NULL	0	NULL	 mechanism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of the timing of labeling and mitotic index peaks by different parameters of the LD cycle suggests a mechanism for cell cycle regulation by the environmental lighting schedule .
	manualset3
252946	8	425735	7	NULL	NULL	0	NULL	cell cycle regulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of the timing of labeling and mitotic index peaks by different parameters of the LD cycle suggests a mechanism for cell cycle regulation by the environmental lighting schedule .
	manualset3
252947	9	425735	7	NULL	NULL	0	NULL	environmental lighting schedule	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of the timing of labeling and mitotic index peaks by different parameters of the LD cycle suggests a mechanism for cell cycle regulation by the environmental lighting schedule .
	manualset3
252948	1	425736	7	NULL	NULL	0	NULL	Control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of tsetse flies using insecticide-treated targets is often hampered by vegetation re-growth and encroachment which obscures a target and renders it less effective .
	manualset3
252949	2	425736	7	NULL	NULL	0	NULL	tsetse flies	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of tsetse flies using insecticide-treated targets is often hampered by vegetation re-growth and encroachment which obscures a target and renders it less effective .
	manualset3
252950	3	425736	7	NULL	NULL	0	NULL	 insecticide-treated targets	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of tsetse flies using insecticide-treated targets is often hampered by vegetation re-growth and encroachment which obscures a target and renders it less effective .
	manualset3
252951	4	425736	7	NULL	NULL	0	NULL	vegetation re-growth 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of tsetse flies using insecticide-treated targets is often hampered by vegetation re-growth and encroachment which obscures a target and renders it less effective .
	manualset3
252952	5	425736	7	NULL	NULL	0	NULL	 encroachment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of tsetse flies using insecticide-treated targets is often hampered by vegetation re-growth and encroachment which obscures a target and renders it less effective .
	manualset3
252953	6	425736	7	NULL	NULL	0	NULL	 target 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Control of tsetse flies using insecticide-treated targets is often hampered by vegetation re-growth and encroachment which obscures a target and renders it less effective .
	manualset3
252954	1	425737	7	NULL	NULL	0	NULL	Control patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Control patients were matched to case patients for ethnicity , age , and week of visit .
	manualset3
252955	2	425737	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Control patients were matched to case patients for ethnicity , age , and week of visit .
	manualset3
252956	3	425737	7	NULL	NULL	0	NULL	ethnicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Control patients were matched to case patients for ethnicity , age , and week of visit .
	manualset3
252957	4	425737	7	NULL	NULL	0	NULL	age	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Control patients were matched to case patients for ethnicity , age , and week of visit .
	manualset3
252958	5	425737	7	NULL	NULL	NULL	NULL	week	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Control patients were matched to case patients for ethnicity , age , and week of visit .
	manualset3
256613	6	425737	7	NULL	NULL	NULL	NULL	visit	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Control patients were matched to case patients for ethnicity , age , and week of visit .
	manualset3
252959	1	425738	7	NULL	NULL	0	NULL	Control tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Control tissues displayed a reproducible response to bethanechol stimulation at different calcium concentrations with an ED50 of 0.4 mM calcium and a peak response of 5.0 + / -0.4 grams tension .
	manualset3
252960	2	425738	7	NULL	NULL	0	NULL	 reproducible response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Control tissues displayed a reproducible response to bethanechol stimulation at different calcium concentrations with an ED50 of 0.4 mM calcium and a peak response of 5.0 + / -0.4 grams tension .
	manualset3
252961	3	425738	7	NULL	NULL	0	NULL	bethanechol stimulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Control tissues displayed a reproducible response to bethanechol stimulation at different calcium concentrations with an ED50 of 0.4 mM calcium and a peak response of 5.0 + / -0.4 grams tension .
	manualset3
252962	4	425738	7	NULL	NULL	0	NULL	different calcium concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Control tissues displayed a reproducible response to bethanechol stimulation at different calcium concentrations with an ED50 of 0.4 mM calcium and a peak response of 5.0 + / -0.4 grams tension .
	manualset3
252963	5	425738	7	NULL	NULL	0	NULL	ED50	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Control tissues displayed a reproducible response to bethanechol stimulation at different calcium concentrations with an ED50 of 0.4 mM calcium and a peak response of 5.0 + / -0.4 grams tension .
	manualset3
252964	6	425738	7	NULL	NULL	0	NULL	 0.4 mM	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Control tissues displayed a reproducible response to bethanechol stimulation at different calcium concentrations with an ED50 of 0.4 mM calcium and a peak response of 5.0 + / -0.4 grams tension .
	manualset3
252965	7	425738	7	NULL	NULL	0	NULL	calcium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Control tissues displayed a reproducible response to bethanechol stimulation at different calcium concentrations with an ED50 of 0.4 mM calcium and a peak response of 5.0 + / -0.4 grams tension .
	manualset3
252966	8	425738	7	NULL	NULL	0	NULL	 peak response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Control tissues displayed a reproducible response to bethanechol stimulation at different calcium concentrations with an ED50 of 0.4 mM calcium and a peak response of 5.0 + / -0.4 grams tension .
	manualset3
252967	9	425738	7	NULL	NULL	0	NULL	5.0 + / -0.4 grams tension	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Control tissues displayed a reproducible response to bethanechol stimulation at different calcium concentrations with an ED50 of 0.4 mM calcium and a peak response of 5.0 + / -0.4 grams tension .
	manualset3
252968	1	425739	7	NULL	NULL	0	NULL	Control variables	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Control variables included age , gender , ethnicity , and acculturation .
	manualset3
252969	2	425739	7	NULL	NULL	0	NULL	age	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Control variables included age , gender , ethnicity , and acculturation .
	manualset3
252970	3	425739	7	NULL	NULL	0	NULL	gender	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Control variables included age , gender , ethnicity , and acculturation .
	manualset3
252971	4	425739	7	NULL	NULL	0	NULL	ethnicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Control variables included age , gender , ethnicity , and acculturation .
	manualset3
252972	5	425739	7	NULL	NULL	0	NULL	acculturation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Control variables included age , gender , ethnicity , and acculturation .
	manualset3
252973	1	425740	7	NULL	NULL	0	NULL	Control vessel diameter 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Control vessel diameter decreased from 5.2 mm + / - 0.3 to 5.1 mm + / - 0.3 ( 2.4 % + / - 1.0 % when standardized to baseline diameter ) and intimal hyperplastic vessels from 6.2 mm + / - 0.4 to 5.7 mm + / - 0.4 ( 7.6 % + / - 1.7 % ) .
	manualset3
252974	2	425740	7	NULL	NULL	NULL	NULL	5.2 mm + / - 0.3	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Control vessel diameter decreased from 5.2 mm + / - 0.3 to 5.1 mm + / - 0.3 ( 2.4 % + / - 1.0 % when standardized to baseline diameter ) and intimal hyperplastic vessels from 6.2 mm + / - 0.4 to 5.7 mm + / - 0.4 ( 7.6 % + / - 1.7 % ) .
	manualset3
252975	3	425740	7	NULL	NULL	NULL	NULL	 5.1 mm + / - 0.3	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Control vessel diameter decreased from 5.2 mm + / - 0.3 to 5.1 mm + / - 0.3 ( 2.4 % + / - 1.0 % when standardized to baseline diameter ) and intimal hyperplastic vessels from 6.2 mm + / - 0.4 to 5.7 mm + / - 0.4 ( 7.6 % + / - 1.7 % ) .
	manualset3
252976	4	425740	7	NULL	NULL	0	NULL	2.4 % + / - 1.0 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Control vessel diameter decreased from 5.2 mm + / - 0.3 to 5.1 mm + / - 0.3 ( 2.4 % + / - 1.0 % when standardized to baseline diameter ) and intimal hyperplastic vessels from 6.2 mm + / - 0.4 to 5.7 mm + / - 0.4 ( 7.6 % + / - 1.7 % ) .
	manualset3
252977	5	425740	7	NULL	NULL	0	NULL	 baseline diameter	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Control vessel diameter decreased from 5.2 mm + / - 0.3 to 5.1 mm + / - 0.3 ( 2.4 % + / - 1.0 % when standardized to baseline diameter ) and intimal hyperplastic vessels from 6.2 mm + / - 0.4 to 5.7 mm + / - 0.4 ( 7.6 % + / - 1.7 % ) .
	manualset3
252978	6	425740	7	NULL	NULL	0	NULL	intimal hyperplastic vessels	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Control vessel diameter decreased from 5.2 mm + / - 0.3 to 5.1 mm + / - 0.3 ( 2.4 % + / - 1.0 % when standardized to baseline diameter ) and intimal hyperplastic vessels from 6.2 mm + / - 0.4 to 5.7 mm + / - 0.4 ( 7.6 % + / - 1.7 % ) .
	manualset3
252979	7	425740	7	NULL	NULL	0	NULL	6.2 mm + / - 0.4 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Control vessel diameter decreased from 5.2 mm + / - 0.3 to 5.1 mm + / - 0.3 ( 2.4 % + / - 1.0 % when standardized to baseline diameter ) and intimal hyperplastic vessels from 6.2 mm + / - 0.4 to 5.7 mm + / - 0.4 ( 7.6 % + / - 1.7 % ) .
	manualset3
252980	8	425740	7	NULL	NULL	0	NULL	 5.7 mm + / - 0.4	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Control vessel diameter decreased from 5.2 mm + / - 0.3 to 5.1 mm + / - 0.3 ( 2.4 % + / - 1.0 % when standardized to baseline diameter ) and intimal hyperplastic vessels from 6.2 mm + / - 0.4 to 5.7 mm + / - 0.4 ( 7.6 % + / - 1.7 % ) .
	manualset3
252981	9	425740	7	NULL	NULL	0	NULL	7.6 % + / - 1.7 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Control vessel diameter decreased from 5.2 mm + / - 0.3 to 5.1 mm + / - 0.3 ( 2.4 % + / - 1.0 % when standardized to baseline diameter ) and intimal hyperplastic vessels from 6.2 mm + / - 0.4 to 5.7 mm + / - 0.4 ( 7.6 % + / - 1.7 % ) .
	manualset3
252982	1	425741	7	NULL	NULL	0	NULL	Controllable water permeation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Controllable water permeation on a poly ( N-isopropylacrylamide ) - modified nanostructured copper mesh film .
	manualset3
252983	2	425741	7	NULL	NULL	0	NULL	 poly ( N-isopropylacrylamide ) - modified nanostructured copper mesh film	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Controllable water permeation on a poly ( N-isopropylacrylamide ) - modified nanostructured copper mesh film .
	manualset3
252984	1	425742	7	NULL	NULL	0	NULL	Controlled entry	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlled entry into the intralumenal vesicles of multivesicular bodies plays a key role in the recycling of secretory granule membrane proteins .
	manualset3
252985	2	425742	7	NULL	NULL	0	NULL	 intralumenal vesicles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlled entry into the intralumenal vesicles of multivesicular bodies plays a key role in the recycling of secretory granule membrane proteins .
	manualset3
252986	3	425742	7	NULL	NULL	0	NULL	multivesicular bodies	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlled entry into the intralumenal vesicles of multivesicular bodies plays a key role in the recycling of secretory granule membrane proteins .
	manualset3
252987	4	425742	7	NULL	NULL	0	NULL	key role 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlled entry into the intralumenal vesicles of multivesicular bodies plays a key role in the recycling of secretory granule membrane proteins .
	manualset3
252988	5	425742	7	NULL	NULL	0	NULL	 recycling	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlled entry into the intralumenal vesicles of multivesicular bodies plays a key role in the recycling of secretory granule membrane proteins .
	manualset3
252989	6	425742	7	NULL	NULL	0	NULL	secretory granule membrane proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlled entry into the intralumenal vesicles of multivesicular bodies plays a key role in the recycling of secretory granule membrane proteins .
	manualset3
252990	1	425743	7	NULL	NULL	0	NULL	Controlled lysosomal rupture	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlled lysosomal rupture was initiated in lysosome-rich , macrophage-like cells by the synthetic lysosomotropic detergent , O-methyl-serine dodecylamide hydrochloride ( MSDH ) .
	manualset3
252991	2	425743	7	NULL	NULL	0	NULL	lysosome-rich , macrophage-like cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlled lysosomal rupture was initiated in lysosome-rich , macrophage-like cells by the synthetic lysosomotropic detergent , O-methyl-serine dodecylamide hydrochloride ( MSDH ) .
	manualset3
252992	3	425743	7	NULL	NULL	0	NULL	synthetic lysosomotropic detergent	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlled lysosomal rupture was initiated in lysosome-rich , macrophage-like cells by the synthetic lysosomotropic detergent , O-methyl-serine dodecylamide hydrochloride ( MSDH ) .
	manualset3
252993	4	425743	7	NULL	NULL	0	NULL	O-methyl-serine dodecylamide hydrochloride ( MSDH )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlled lysosomal rupture was initiated in lysosome-rich , macrophage-like cells by the synthetic lysosomotropic detergent , O-methyl-serine dodecylamide hydrochloride ( MSDH ) .
	manualset3
252994	1	425744	7	NULL	NULL	0	NULL	Low-dose adenosine echocardiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Low-dose adenosine echocardiography for detection of myocardial viability in patients with acute myocardial infarction . ) .
	manualset3
252995	2	425744	7	NULL	NULL	0	NULL	detection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Low-dose adenosine echocardiography for detection of myocardial viability in patients with acute myocardial infarction . ) .
	manualset3
252996	3	425744	7	NULL	NULL	0	NULL	myocardial viability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Low-dose adenosine echocardiography for detection of myocardial viability in patients with acute myocardial infarction . ) .
	manualset3
252997	4	425744	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Low-dose adenosine echocardiography for detection of myocardial viability in patients with acute myocardial infarction . ) .
	manualset3
252998	5	425744	7	NULL	NULL	0	NULL	acute myocardial infarction	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Low-dose adenosine echocardiography for detection of myocardial viability in patients with acute myocardial infarction . ) .
	manualset3
252999	1	425745	7	NULL	NULL	0	NULL	Controlled studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlled studies of chimpanzee cultural transmission .
	manualset3
253000	2	425745	7	NULL	NULL	0	NULL	chimpanzee cultural transmission	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlled studies of chimpanzee cultural transmission .
	manualset3
253001	1	425746	7	NULL	NULL	0	NULL	Controlled trial	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlled trial of azathioprine and plasma exchange in addition to prednisolone in the treatment of bullous pemphigoid .
	manualset3
253002	2	425746	7	NULL	NULL	0	NULL	azathioprine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlled trial of azathioprine and plasma exchange in addition to prednisolone in the treatment of bullous pemphigoid .
	manualset3
253003	3	425746	7	NULL	NULL	0	NULL	plasma exchange	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlled trial of azathioprine and plasma exchange in addition to prednisolone in the treatment of bullous pemphigoid .
	manualset3
253004	4	425746	7	NULL	NULL	0	NULL	prednisolone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlled trial of azathioprine and plasma exchange in addition to prednisolone in the treatment of bullous pemphigoid .
	manualset3
253005	5	425746	7	NULL	NULL	0	NULL	 treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlled trial of azathioprine and plasma exchange in addition to prednisolone in the treatment of bullous pemphigoid .
	manualset3
253006	6	425746	7	NULL	NULL	0	NULL	bullous pemphigoid	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlled trial of azathioprine and plasma exchange in addition to prednisolone in the treatment of bullous pemphigoid .
	manualset3
253007	1	425747	7	NULL	NULL	0	NULL	blood glucose level 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlling blood glucose level for diabetic patients can be accomplished by using several methods , such as life style modification , oral medication , and insulin .
	manualset3
253008	2	425747	7	NULL	NULL	0	NULL	diabetic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlling blood glucose level for diabetic patients can be accomplished by using several methods , such as life style modification , oral medication , and insulin .
	manualset3
253009	3	425747	7	NULL	NULL	0	NULL	several methods	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlling blood glucose level for diabetic patients can be accomplished by using several methods , such as life style modification , oral medication , and insulin .
	manualset3
253010	4	425747	7	NULL	NULL	0	NULL	life style modification	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlling blood glucose level for diabetic patients can be accomplished by using several methods , such as life style modification , oral medication , and insulin .
	manualset3
253011	5	425747	7	NULL	NULL	0	NULL	 oral medication	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlling blood glucose level for diabetic patients can be accomplished by using several methods , such as life style modification , oral medication , and insulin .
	manualset3
253012	6	425747	7	NULL	NULL	0	NULL	 insulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlling blood glucose level for diabetic patients can be accomplished by using several methods , such as life style modification , oral medication , and insulin .
	manualset3
253013	7	425747	7	NULL	NULL	0	NULL	Controlling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlling blood glucose level for diabetic patients can be accomplished by using several methods , such as life style modification , oral medication , and insulin .
	manualset3
253014	1	425748	7	NULL	NULL	0	NULL	Controlling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlling for gender , grade in school , prior academic achievement , and level of intelligence , we used path analysis to examine the longitudinal relations between overestimations of one 's personal agency and subsequent school performance .
	manualset3
253015	2	425748	7	NULL	NULL	0	NULL	gender	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlling for gender , grade in school , prior academic achievement , and level of intelligence , we used path analysis to examine the longitudinal relations between overestimations of one 's personal agency and subsequent school performance .
	manualset3
253016	3	425748	7	NULL	NULL	0	NULL	grade in school	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlling for gender , grade in school , prior academic achievement , and level of intelligence , we used path analysis to examine the longitudinal relations between overestimations of one 's personal agency and subsequent school performance .
	manualset3
253017	4	425748	7	NULL	NULL	0	NULL	academic achievement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlling for gender , grade in school , prior academic achievement , and level of intelligence , we used path analysis to examine the longitudinal relations between overestimations of one 's personal agency and subsequent school performance .
	manualset3
253018	5	425748	7	NULL	NULL	0	NULL	level of intelligence	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlling for gender , grade in school , prior academic achievement , and level of intelligence , we used path analysis to examine the longitudinal relations between overestimations of one 's personal agency and subsequent school performance .
	manualset3
253019	6	425748	7	NULL	NULL	0	NULL	path analysis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlling for gender , grade in school , prior academic achievement , and level of intelligence , we used path analysis to examine the longitudinal relations between overestimations of one 's personal agency and subsequent school performance .
	manualset3
253020	7	425748	7	NULL	NULL	0	NULL	longitudinal relations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlling for gender , grade in school , prior academic achievement , and level of intelligence , we used path analysis to examine the longitudinal relations between overestimations of one 's personal agency and subsequent school performance .
	manualset3
253021	8	425748	7	NULL	NULL	0	NULL	 overestimations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlling for gender , grade in school , prior academic achievement , and level of intelligence , we used path analysis to examine the longitudinal relations between overestimations of one 's personal agency and subsequent school performance .
	manualset3
253022	9	425748	7	NULL	NULL	0	NULL	one 's personal agency	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlling for gender , grade in school , prior academic achievement , and level of intelligence , we used path analysis to examine the longitudinal relations between overestimations of one 's personal agency and subsequent school performance .
	manualset3
253023	10	425748	7	NULL	NULL	0	NULL	school performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlling for gender , grade in school , prior academic achievement , and level of intelligence , we used path analysis to examine the longitudinal relations between overestimations of one 's personal agency and subsequent school performance .
	manualset3
253024	1	425749	7	NULL	NULL	0	NULL	Controlling hemoptysis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlling hemoptysis : An alternative approach .
	manualset3
253025	2	425749	7	NULL	NULL	0	NULL	alternative approach	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Controlling hemoptysis : An alternative approach .
	manualset3
253026	1	425750	7	NULL	NULL	0	NULL	Controls	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Controls comprised three groups of ICR newborn mice : normal , ( 100 ) ginseng , ( 200 ) , and vehicle ( 316 ) .
	manualset3
253027	2	425750	7	NULL	NULL	0	NULL	three groups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Controls comprised three groups of ICR newborn mice : normal , ( 100 ) ginseng , ( 200 ) , and vehicle ( 316 ) .
	manualset3
253028	3	425750	7	NULL	NULL	0	NULL	ICR newborn mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Controls comprised three groups of ICR newborn mice : normal , ( 100 ) ginseng , ( 200 ) , and vehicle ( 316 ) .
	manualset3
253029	4	425750	7	NULL	NULL	0	NULL	normal 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Controls comprised three groups of ICR newborn mice : normal , ( 100 ) ginseng , ( 200 ) , and vehicle ( 316 ) .
	manualset3
253030	5	425750	7	NULL	NULL	NULL	NULL	100	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Controls comprised three groups of ICR newborn mice : normal , ( 100 ) ginseng , ( 200 ) , and vehicle ( 316 ) .
	manualset3
253031	6	425750	7	NULL	NULL	0	NULL	ginseng	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Controls comprised three groups of ICR newborn mice : normal , ( 100 ) ginseng , ( 200 ) , and vehicle ( 316 ) .
	manualset3
253032	7	425750	7	NULL	NULL	0	NULL	 200	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Controls comprised three groups of ICR newborn mice : normal , ( 100 ) ginseng , ( 200 ) , and vehicle ( 316 ) .
	manualset3
253033	8	425750	7	NULL	NULL	0	NULL	 vehicle 	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Controls comprised three groups of ICR newborn mice : normal , ( 100 ) ginseng , ( 200 ) , and vehicle ( 316 ) .
	manualset3
253034	9	425750	7	NULL	NULL	0	NULL	 316	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Controls comprised three groups of ICR newborn mice : normal , ( 100 ) ginseng , ( 200 ) , and vehicle ( 316 ) .
	manualset3
253035	1	425751	7	NULL	NULL	0	NULL	Controls	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Controls with no ethanol showed no change in the frequency of the AdhF isoallele .
	manualset3
253036	2	425751	7	NULL	NULL	0	NULL	ethanol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Controls with no ethanol showed no change in the frequency of the AdhF isoallele .
	manualset3
253037	3	425751	7	NULL	NULL	0	NULL	change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Controls with no ethanol showed no change in the frequency of the AdhF isoallele .
	manualset3
253038	4	425751	7	NULL	NULL	0	NULL	frequency	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Controls with no ethanol showed no change in the frequency of the AdhF isoallele .
	manualset3
253039	5	425751	7	NULL	NULL	0	NULL	AdhF isoallele	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Controls with no ethanol showed no change in the frequency of the AdhF isoallele .
	manualset3
253040	1	425752	7	NULL	NULL	0	NULL	Lung changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Lung changes in recurrent tuberculosis of the eye in patients receiving antibacterial preparations ) .
	manualset3
253041	2	425752	7	NULL	NULL	0	NULL	recurrent tuberculosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Lung changes in recurrent tuberculosis of the eye in patients receiving antibacterial preparations ) .
	manualset3
253042	3	425752	7	NULL	NULL	0	NULL	eye	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Lung changes in recurrent tuberculosis of the eye in patients receiving antibacterial preparations ) .
	manualset3
253043	4	425752	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Lung changes in recurrent tuberculosis of the eye in patients receiving antibacterial preparations ) .
	manualset3
253044	5	425752	7	NULL	NULL	0	NULL	antibacterial preparations	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	( Lung changes in recurrent tuberculosis of the eye in patients receiving antibacterial preparations ) .
	manualset3
253045	1	425753	7	NULL	NULL	0	NULL	Convection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Convection from the tube to its surroundings is inhibited , but not diffusion .
	manualset3
253046	2	425753	7	NULL	NULL	NULL	NULL	tube	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Convection from the tube to its surroundings is inhibited , but not diffusion .
	manualset3
253047	3	425753	7	NULL	NULL	0	NULL	 surroundings	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Convection from the tube to its surroundings is inhibited , but not diffusion .
	manualset3
253048	4	425753	7	NULL	NULL	0	NULL	diffusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Convection from the tube to its surroundings is inhibited , but not diffusion .
	manualset3
253049	1	425754	7	NULL	NULL	0	NULL	Conventional sensitivity encoding ( SENSE ) reconstruction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conventional sensitivity encoding ( SENSE ) reconstruction is based on equations in the complex domain .
	manualset3
253050	2	425754	7	NULL	NULL	0	NULL	equations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conventional sensitivity encoding ( SENSE ) reconstruction is based on equations in the complex domain .
	manualset3
253051	3	425754	7	NULL	NULL	0	NULL	complex domain	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conventional sensitivity encoding ( SENSE ) reconstruction is based on equations in the complex domain .
	manualset3
253052	1	425755	7	NULL	NULL	0	NULL	Conventional susceptibility testing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Conventional susceptibility testing for the front-line tuberculosis drug pyrazinamide ( PZA ) is difficult , because of the requirement for acid pH for the drug to show activity .
	manualset3
253053	2	425755	7	NULL	NULL	0	NULL	front-line tuberculosis drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Conventional susceptibility testing for the front-line tuberculosis drug pyrazinamide ( PZA ) is difficult , because of the requirement for acid pH for the drug to show activity .
	manualset3
253054	3	425755	7	NULL	NULL	0	NULL	pyrazinamide ( PZA )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Conventional susceptibility testing for the front-line tuberculosis drug pyrazinamide ( PZA ) is difficult , because of the requirement for acid pH for the drug to show activity .
	manualset3
253055	4	425755	7	NULL	NULL	0	NULL	requirement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conventional susceptibility testing for the front-line tuberculosis drug pyrazinamide ( PZA ) is difficult , because of the requirement for acid pH for the drug to show activity .
	manualset3
253056	5	425755	7	NULL	NULL	0	NULL	 acid pH 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Conventional susceptibility testing for the front-line tuberculosis drug pyrazinamide ( PZA ) is difficult , because of the requirement for acid pH for the drug to show activity .
	manualset3
253057	6	425755	7	NULL	NULL	0	NULL	drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Conventional susceptibility testing for the front-line tuberculosis drug pyrazinamide ( PZA ) is difficult , because of the requirement for acid pH for the drug to show activity .
	manualset3
253058	7	425755	7	NULL	NULL	0	NULL	activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Conventional susceptibility testing for the front-line tuberculosis drug pyrazinamide ( PZA ) is difficult , because of the requirement for acid pH for the drug to show activity .
	manualset3
253059	1	425756	7	NULL	NULL	0	NULL	culture medium	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Conventionally , culture medium is supplemented with fetal bovine serum ( FBS ) : such serum presents potential risks of foreign protein contamination and transmission of viral or prion-related disease if used in culture of cells intended for human reimplantation .
	manualset3
253060	2	425756	7	NULL	NULL	0	NULL	fetal bovine serum ( FBS )	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Conventionally , culture medium is supplemented with fetal bovine serum ( FBS ) : such serum presents potential risks of foreign protein contamination and transmission of viral or prion-related disease if used in culture of cells intended for human reimplantation .
	manualset3
253061	3	425756	7	NULL	NULL	0	NULL	serum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Conventionally , culture medium is supplemented with fetal bovine serum ( FBS ) : such serum presents potential risks of foreign protein contamination and transmission of viral or prion-related disease if used in culture of cells intended for human reimplantation .
	manualset3
253062	4	425756	7	NULL	NULL	0	NULL	potential risks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conventionally , culture medium is supplemented with fetal bovine serum ( FBS ) : such serum presents potential risks of foreign protein contamination and transmission of viral or prion-related disease if used in culture of cells intended for human reimplantation .
	manualset3
253063	5	425756	7	NULL	NULL	0	NULL	foreign protein contamination	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conventionally , culture medium is supplemented with fetal bovine serum ( FBS ) : such serum presents potential risks of foreign protein contamination and transmission of viral or prion-related disease if used in culture of cells intended for human reimplantation .
	manualset3
253064	6	425756	7	NULL	NULL	0	NULL	transmission	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conventionally , culture medium is supplemented with fetal bovine serum ( FBS ) : such serum presents potential risks of foreign protein contamination and transmission of viral or prion-related disease if used in culture of cells intended for human reimplantation .
	manualset3
253065	7	425756	7	NULL	NULL	0	NULL	viral related disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Conventionally , culture medium is supplemented with fetal bovine serum ( FBS ) : such serum presents potential risks of foreign protein contamination and transmission of viral or prion-related disease if used in culture of cells intended for human reimplantation .
	manualset3
253066	8	425756	7	NULL	NULL	0	NULL	prion-related disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Conventionally , culture medium is supplemented with fetal bovine serum ( FBS ) : such serum presents potential risks of foreign protein contamination and transmission of viral or prion-related disease if used in culture of cells intended for human reimplantation .
	manualset3
253067	9	425756	7	NULL	NULL	0	NULL	 culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Conventionally , culture medium is supplemented with fetal bovine serum ( FBS ) : such serum presents potential risks of foreign protein contamination and transmission of viral or prion-related disease if used in culture of cells intended for human reimplantation .
	manualset3
253068	10	425756	7	NULL	NULL	0	NULL	 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Conventionally , culture medium is supplemented with fetal bovine serum ( FBS ) : such serum presents potential risks of foreign protein contamination and transmission of viral or prion-related disease if used in culture of cells intended for human reimplantation .
	manualset3
253069	11	425756	7	NULL	NULL	0	NULL	human reimplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Conventionally , culture medium is supplemented with fetal bovine serum ( FBS ) : such serum presents potential risks of foreign protein contamination and transmission of viral or prion-related disease if used in culture of cells intended for human reimplantation .
	manualset3
253070	1	425757	7	NULL	NULL	NULL	NULL	Convergent syntheses	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Convergent syntheses of di - , tri , tetra - , penta - , and hexa-saccharide allyl glycosides corresponding to the beta-hemolytic Streptococcus Group A cell-wall polysaccharide are described .
	manualset3
253071	2	425757	7	NULL	NULL	NULL	NULL	di-saccharide allyl glycosides	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Convergent syntheses of di - , tri , tetra - , penta - , and hexa-saccharide allyl glycosides corresponding to the beta-hemolytic Streptococcus Group A cell-wall polysaccharide are described .
	manualset3
253072	3	425757	7	NULL	NULL	0	NULL	trisaccharide allyl glycosides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Convergent syntheses of di - , tri , tetra - , penta - , and hexa-saccharide allyl glycosides corresponding to the beta-hemolytic Streptococcus Group A cell-wall polysaccharide are described .
	manualset3
253073	4	425757	7	NULL	NULL	0	NULL	tetra-saccharide allyl glycosides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Convergent syntheses of di - , tri , tetra - , penta - , and hexa-saccharide allyl glycosides corresponding to the beta-hemolytic Streptococcus Group A cell-wall polysaccharide are described .
	manualset3
253074	5	425757	7	NULL	NULL	0	NULL	penta -saccharide allyl glycosides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Convergent syntheses of di - , tri , tetra - , penta - , and hexa-saccharide allyl glycosides corresponding to the beta-hemolytic Streptococcus Group A cell-wall polysaccharide are described .
	manualset3
253075	6	425757	7	NULL	NULL	0	NULL	hexa-saccharide allyl glycosides	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Convergent syntheses of di - , tri , tetra - , penta - , and hexa-saccharide allyl glycosides corresponding to the beta-hemolytic Streptococcus Group A cell-wall polysaccharide are described .
	manualset3
253076	7	425757	7	NULL	NULL	0	NULL	 beta-hemolytic Streptococcus Group A cell-wall polysaccharide	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Convergent syntheses of di - , tri , tetra - , penta - , and hexa-saccharide allyl glycosides corresponding to the beta-hemolytic Streptococcus Group A cell-wall polysaccharide are described .
	manualset3
253077	1	425758	7	NULL	NULL	0	NULL	Converging evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Converging evidence suggests that the representation of visual scenes is much more schematic and abstract than our immediate experience would indicate .
	manualset3
253078	2	425758	7	NULL	NULL	0	NULL	representation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Converging evidence suggests that the representation of visual scenes is much more schematic and abstract than our immediate experience would indicate .
	manualset3
253079	3	425758	7	NULL	NULL	0	NULL	visual scenes	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Converging evidence suggests that the representation of visual scenes is much more schematic and abstract than our immediate experience would indicate .
	manualset3
253080	4	425758	7	NULL	NULL	NULL	NULL	experience	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Converging evidence suggests that the representation of visual scenes is much more schematic and abstract than our immediate experience would indicate .
	manualset3
253081	1	425759	7	NULL	NULL	0	NULL	APZ tumors	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , APZ tumors were more commonly localized within the apical one third of the prostate .
	manualset3
253082	2	425759	7	NULL	NULL	0	NULL	apical one third	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , APZ tumors were more commonly localized within the apical one third of the prostate .
	manualset3
253083	3	425759	7	NULL	NULL	0	NULL	 prostate	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , APZ tumors were more commonly localized within the apical one third of the prostate .
	manualset3
253084	1	425760	7	NULL	NULL	0	NULL	BC-MAD	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , BC-MAD was ineffective in the bar test and improved stepping activity in the drag test to a much lower degree than those achieved with the other preparations .
	manualset3
253085	2	425760	7	NULL	NULL	0	NULL	bar test 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , BC-MAD was ineffective in the bar test and improved stepping activity in the drag test to a much lower degree than those achieved with the other preparations .
	manualset3
253086	3	425760	7	NULL	NULL	0	NULL	stepping activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , BC-MAD was ineffective in the bar test and improved stepping activity in the drag test to a much lower degree than those achieved with the other preparations .
	manualset3
253087	4	425760	7	NULL	NULL	0	NULL	 drag test	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , BC-MAD was ineffective in the bar test and improved stepping activity in the drag test to a much lower degree than those achieved with the other preparations .
	manualset3
253088	5	425760	7	NULL	NULL	0	NULL	lower degree	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , BC-MAD was ineffective in the bar test and improved stepping activity in the drag test to a much lower degree than those achieved with the other preparations .
	manualset3
253089	6	425760	7	NULL	NULL	0	NULL	preparations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , BC-MAD was ineffective in the bar test and improved stepping activity in the drag test to a much lower degree than those achieved with the other preparations .
	manualset3
253090	1	425761	7	NULL	NULL	0	NULL	PPG 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , PPG decreased phosphorylation of IB kinase and IB degradation .
	manualset3
253091	2	425761	7	NULL	NULL	0	NULL	 phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , PPG decreased phosphorylation of IB kinase and IB degradation .
	manualset3
253092	3	425761	7	NULL	NULL	0	NULL	 IB kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , PPG decreased phosphorylation of IB kinase and IB degradation .
	manualset3
253093	4	425761	7	NULL	NULL	0	NULL	 IB degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , PPG decreased phosphorylation of IB kinase and IB degradation .
	manualset3
253094	1	425762	7	NULL	NULL	0	NULL	 Luxation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Luxation of the lens remnants in the vitreous body during phacoemulsification ) .
	manualset3
253095	2	425762	7	NULL	NULL	0	NULL	lens remnants 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Luxation of the lens remnants in the vitreous body during phacoemulsification ) .
	manualset3
253096	3	425762	7	NULL	NULL	0	NULL	vitreous body 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Luxation of the lens remnants in the vitreous body during phacoemulsification ) .
	manualset3
253097	4	425762	7	NULL	NULL	0	NULL	phacoemulsification	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Luxation of the lens remnants in the vitreous body during phacoemulsification ) .
	manualset3
253098	1	425763	7	NULL	NULL	0	NULL	addition 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , after addition of the NO-generating compound NOC-18 , IL-1beta and IL-1alpha concentrations in supernatants were dose-dependently reduced .
	manualset3
253099	2	425763	7	NULL	NULL	0	NULL	NO-generating compound NOC-18	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , after addition of the NO-generating compound NOC-18 , IL-1beta and IL-1alpha concentrations in supernatants were dose-dependently reduced .
	manualset3
253100	3	425763	7	NULL	NULL	0	NULL	IL-1beta concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , after addition of the NO-generating compound NOC-18 , IL-1beta and IL-1alpha concentrations in supernatants were dose-dependently reduced .
	manualset3
253101	4	425763	7	NULL	NULL	0	NULL	IL-1alpha concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , after addition of the NO-generating compound NOC-18 , IL-1beta and IL-1alpha concentrations in supernatants were dose-dependently reduced .
	manualset3
253102	5	425763	7	NULL	NULL	0	NULL	 supernatants	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , after addition of the NO-generating compound NOC-18 , IL-1beta and IL-1alpha concentrations in supernatants were dose-dependently reduced .
	manualset3
253103	1	425764	7	NULL	NULL	0	NULL	facial-skeletal abnormalities 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , correcting facial-skeletal abnormalities have been found to alleviate many medical problems , such as chronic headaches , neck-back-shoulder pain , respiratory disorders , auditory disorders , etc. .
	manualset3
253104	2	425764	7	NULL	NULL	0	NULL	medical problems 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , correcting facial-skeletal abnormalities have been found to alleviate many medical problems , such as chronic headaches , neck-back-shoulder pain , respiratory disorders , auditory disorders , etc. .
	manualset3
253105	3	425764	7	NULL	NULL	0	NULL	chronic headaches	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , correcting facial-skeletal abnormalities have been found to alleviate many medical problems , such as chronic headaches , neck-back-shoulder pain , respiratory disorders , auditory disorders , etc. .
	manualset3
253106	4	425764	7	NULL	NULL	0	NULL	neck-back-shoulder pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , correcting facial-skeletal abnormalities have been found to alleviate many medical problems , such as chronic headaches , neck-back-shoulder pain , respiratory disorders , auditory disorders , etc. .
	manualset3
253107	5	425764	7	NULL	NULL	0	NULL	respiratory disorders 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , correcting facial-skeletal abnormalities have been found to alleviate many medical problems , such as chronic headaches , neck-back-shoulder pain , respiratory disorders , auditory disorders , etc. .
	manualset3
253108	6	425764	7	NULL	NULL	0	NULL	auditory disorders	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , correcting facial-skeletal abnormalities have been found to alleviate many medical problems , such as chronic headaches , neck-back-shoulder pain , respiratory disorders , auditory disorders , etc. .
	manualset3
253109	1	425765	7	NULL	NULL	0	NULL	biochemist	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , from a biochemist point of view lactate is a good cellular substrate which can be easily converted to pyruvate and used as gluconeogenic substrate , or oxidised or transaminated into alanine .
	manualset3
253110	2	425765	7	NULL	NULL	0	NULL	lactate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , from a biochemist point of view lactate is a good cellular substrate which can be easily converted to pyruvate and used as gluconeogenic substrate , or oxidised or transaminated into alanine .
	manualset3
253111	3	425765	7	NULL	NULL	0	NULL	good cellular substrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , from a biochemist point of view lactate is a good cellular substrate which can be easily converted to pyruvate and used as gluconeogenic substrate , or oxidised or transaminated into alanine .
	manualset3
253112	4	425765	7	NULL	NULL	0	NULL	 pyruvate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , from a biochemist point of view lactate is a good cellular substrate which can be easily converted to pyruvate and used as gluconeogenic substrate , or oxidised or transaminated into alanine .
	manualset3
253113	5	425765	7	NULL	NULL	0	NULL	gluconeogenic substrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , from a biochemist point of view lactate is a good cellular substrate which can be easily converted to pyruvate and used as gluconeogenic substrate , or oxidised or transaminated into alanine .
	manualset3
253114	6	425765	7	NULL	NULL	0	NULL	 alanine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , from a biochemist point of view lactate is a good cellular substrate which can be easily converted to pyruvate and used as gluconeogenic substrate , or oxidised or transaminated into alanine .
	manualset3
253161	1	425766	7	NULL	NULL	0	NULL	 lipid 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , lipid , once incorporated into the basal discs , diffuses throughout the entire ROS as evidenced by an exponential decline in specific radioactivity .
	manualset3
253162	2	425766	7	NULL	NULL	0	NULL	basal discs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , lipid , once incorporated into the basal discs , diffuses throughout the entire ROS as evidenced by an exponential decline in specific radioactivity .
	manualset3
253163	3	425766	7	NULL	NULL	0	NULL	entire ROS	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , lipid , once incorporated into the basal discs , diffuses throughout the entire ROS as evidenced by an exponential decline in specific radioactivity .
	manualset3
253164	4	425766	7	NULL	NULL	0	NULL	exponential decline	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , lipid , once incorporated into the basal discs , diffuses throughout the entire ROS as evidenced by an exponential decline in specific radioactivity .
	manualset3
253165	5	425766	7	NULL	NULL	0	NULL	specific radioactivity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , lipid , once incorporated into the basal discs , diffuses throughout the entire ROS as evidenced by an exponential decline in specific radioactivity .
	manualset3
253166	1	425767	7	NULL	NULL	0	NULL	 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , mice with increased hepatic mTORC1 activity exhibited decreased expression of PCSK9 and increased levels of hepatic LDLR protein levels .
	manualset3
253167	2	425767	7	NULL	NULL	0	NULL	hepatic mTORC1 activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , mice with increased hepatic mTORC1 activity exhibited decreased expression of PCSK9 and increased levels of hepatic LDLR protein levels .
	manualset3
253168	3	425767	7	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , mice with increased hepatic mTORC1 activity exhibited decreased expression of PCSK9 and increased levels of hepatic LDLR protein levels .
	manualset3
253169	4	425767	7	NULL	NULL	0	NULL	PCSK9	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , mice with increased hepatic mTORC1 activity exhibited decreased expression of PCSK9 and increased levels of hepatic LDLR protein levels .
	manualset3
253170	5	425767	7	NULL	NULL	0	NULL	levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , mice with increased hepatic mTORC1 activity exhibited decreased expression of PCSK9 and increased levels of hepatic LDLR protein levels .
	manualset3
253171	6	425767	7	NULL	NULL	0	NULL	hepatic LDLR protein levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , mice with increased hepatic mTORC1 activity exhibited decreased expression of PCSK9 and increased levels of hepatic LDLR protein levels .
	manualset3
253172	1	425768	7	NULL	NULL	0	NULL	 oxidative cross-linking 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , oxidative cross-linking of spectrin by diamide reduced the diffusion coefficients of both membrane and C proteins .
	manualset3
253173	2	425768	7	NULL	NULL	0	NULL	spectrin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , oxidative cross-linking of spectrin by diamide reduced the diffusion coefficients of both membrane and C proteins .
	manualset3
253174	3	425768	7	NULL	NULL	0	NULL	diamide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , oxidative cross-linking of spectrin by diamide reduced the diffusion coefficients of both membrane and C proteins .
	manualset3
253175	4	425768	7	NULL	NULL	0	NULL	diffusion coefficients	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , oxidative cross-linking of spectrin by diamide reduced the diffusion coefficients of both membrane and C proteins .
	manualset3
253176	5	425768	7	NULL	NULL	0	NULL	membrane proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , oxidative cross-linking of spectrin by diamide reduced the diffusion coefficients of both membrane and C proteins .
	manualset3
253177	6	425768	7	NULL	NULL	0	NULL	C proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , oxidative cross-linking of spectrin by diamide reduced the diffusion coefficients of both membrane and C proteins .
	manualset3
253178	1	425769	7	NULL	NULL	0	NULL	killing	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , the killing of splenic T cells by specific heterologous antiserum directed against rabbit thymus lymphocyte antigen abolished the enhancement .
	manualset3
253179	2	425769	7	NULL	NULL	0	NULL	splenic T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , the killing of splenic T cells by specific heterologous antiserum directed against rabbit thymus lymphocyte antigen abolished the enhancement .
	manualset3
253180	3	425769	7	NULL	NULL	0	NULL	heterologous antiserum	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , the killing of splenic T cells by specific heterologous antiserum directed against rabbit thymus lymphocyte antigen abolished the enhancement .
	manualset3
253181	4	425769	7	NULL	NULL	0	NULL	rabbit thymus lymphocyte antigen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , the killing of splenic T cells by specific heterologous antiserum directed against rabbit thymus lymphocyte antigen abolished the enhancement .
	manualset3
253182	5	425769	7	NULL	NULL	0	NULL	enhancement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , the killing of splenic T cells by specific heterologous antiserum directed against rabbit thymus lymphocyte antigen abolished the enhancement .
	manualset3
253183	1	425770	7	NULL	NULL	NULL	NULL	Changes	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Conversely , there were no significant changes in reference-segment EEM or plaque areas in the Cypher group .
	manualset3
253184	2	425770	7	NULL	NULL	0	NULL	reference-segment EEM	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , there were no significant changes in reference-segment EEM or plaque areas in the Cypher group .
	manualset3
253185	3	425770	7	NULL	NULL	0	NULL	plaque areas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , there were no significant changes in reference-segment EEM or plaque areas in the Cypher group .
	manualset3
253186	4	425770	7	NULL	NULL	0	NULL	Cypher group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely , there were no significant changes in reference-segment EEM or plaque areas in the Cypher group .
	manualset3
253187	1	425771	7	NULL	NULL	0	NULL	fully dephosphorylated peptide SSSEESIT	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely the fully dephosphorylated peptide SSSEESIT is not affected by CK-1 to any detectable extent and its glutamyl derivative EEEEESIT displays a more than 50-fold higher Km and a 5-fold lower Vmax as compared to the parent phosphopeptide .
	manualset3
253188	2	425771	7	NULL	NULL	0	NULL	CK-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely the fully dephosphorylated peptide SSSEESIT is not affected by CK-1 to any detectable extent and its glutamyl derivative EEEEESIT displays a more than 50-fold higher Km and a 5-fold lower Vmax as compared to the parent phosphopeptide .
	manualset3
253190	4	425771	7	NULL	NULL	0	NULL	 glutamyl derivative EEEEESIT 	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely the fully dephosphorylated peptide SSSEESIT is not affected by CK-1 to any detectable extent and its glutamyl derivative EEEEESIT displays a more than 50-fold higher Km and a 5-fold lower Vmax as compared to the parent phosphopeptide .
	manualset3
253191	5	425771	7	NULL	NULL	0	NULL	 50-fold higher Km	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely the fully dephosphorylated peptide SSSEESIT is not affected by CK-1 to any detectable extent and its glutamyl derivative EEEEESIT displays a more than 50-fold higher Km and a 5-fold lower Vmax as compared to the parent phosphopeptide .
	manualset3
253192	6	425771	7	NULL	NULL	0	NULL	5-fold lower Vmax 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely the fully dephosphorylated peptide SSSEESIT is not affected by CK-1 to any detectable extent and its glutamyl derivative EEEEESIT displays a more than 50-fold higher Km and a 5-fold lower Vmax as compared to the parent phosphopeptide .
	manualset3
253193	7	425771	7	NULL	NULL	0	NULL	parent phosphopeptide	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversely the fully dephosphorylated peptide SSSEESIT is not affected by CK-1 to any detectable extent and its glutamyl derivative EEEEESIT displays a more than 50-fold higher Km and a 5-fold lower Vmax as compared to the parent phosphopeptide .
	manualset3
253194	1	425772	7	NULL	NULL	0	NULL	Conversion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversion of CHF3 to CH2 = CF2 via reaction with CH4 and CaBr2 .
	manualset3
253195	2	425772	7	NULL	NULL	0	NULL	CHF3 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversion of CHF3 to CH2 = CF2 via reaction with CH4 and CaBr2 .
	manualset3
253197	3	425772	7	NULL	NULL	0	NULL	 CH2 = CF2	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversion of CHF3 to CH2 = CF2 via reaction with CH4 and CaBr2 .
	manualset3
253198	4	425772	7	NULL	NULL	0	NULL	reaction 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversion of CHF3 to CH2 = CF2 via reaction with CH4 and CaBr2 .
	manualset3
253199	5	425772	7	NULL	NULL	0	NULL	CH4	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversion of CHF3 to CH2 = CF2 via reaction with CH4 and CaBr2 .
	manualset3
253200	6	425772	7	NULL	NULL	0	NULL	CaBr2 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversion of CHF3 to CH2 = CF2 via reaction with CH4 and CaBr2 .
	manualset3
253204	1	425773	7	NULL	NULL	0	NULL	Conversion 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversion to SR was verified by 24-hour Holter monitoring .
	manualset3
253205	2	425773	7	NULL	NULL	0	NULL	SR	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversion to SR was verified by 24-hour Holter monitoring .
	manualset3
253206	3	425773	7	NULL	NULL	0	NULL	24-hour	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversion to SR was verified by 24-hour Holter monitoring .
	manualset3
253207	4	425773	7	NULL	NULL	0	NULL	Holter monitoring	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversion to SR was verified by 24-hour Holter monitoring .
	manualset3
253208	1	425774	7	NULL	NULL	NULL	NULL	Conversion	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Conversion to TAC OD is safe , enhances immunosuppressant adherence and should be accompanied by a close TAC level monitoring during the initial period .
	manualset3
253209	2	425774	7	NULL	NULL	NULL	NULL	TAC OD	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Conversion to TAC OD is safe , enhances immunosuppressant adherence and should be accompanied by a close TAC level monitoring during the initial period .
	manualset3
253210	3	425774	7	NULL	NULL	0	NULL	immunosuppressant adherence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversion to TAC OD is safe , enhances immunosuppressant adherence and should be accompanied by a close TAC level monitoring during the initial period .
	manualset3
253211	4	425774	7	NULL	NULL	0	NULL	TAC level monitoring	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversion to TAC OD is safe , enhances immunosuppressant adherence and should be accompanied by a close TAC level monitoring during the initial period .
	manualset3
253212	5	425774	7	NULL	NULL	0	NULL	initial period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Conversion to TAC OD is safe , enhances immunosuppressant adherence and should be accompanied by a close TAC level monitoring during the initial period .
	manualset3
253213	1	425775	7	NULL	NULL	0	NULL	Cooling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Cooling causes a sharp rise of the pathological mitosis , represented mainly by the forms of pathology connected with the disorganization of the mitotic apparatus , such as C-mitosis and dispersion of chromosomes in the metaphase .
	manualset3
253214	2	425775	7	NULL	NULL	0	NULL	sharp rise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Cooling causes a sharp rise of the pathological mitosis , represented mainly by the forms of pathology connected with the disorganization of the mitotic apparatus , such as C-mitosis and dispersion of chromosomes in the metaphase .
	manualset3
253215	3	425775	7	NULL	NULL	0	NULL	pathological mitosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cooling causes a sharp rise of the pathological mitosis , represented mainly by the forms of pathology connected with the disorganization of the mitotic apparatus , such as C-mitosis and dispersion of chromosomes in the metaphase .
	manualset3
253216	4	425775	7	NULL	NULL	0	NULL	forms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Cooling causes a sharp rise of the pathological mitosis , represented mainly by the forms of pathology connected with the disorganization of the mitotic apparatus , such as C-mitosis and dispersion of chromosomes in the metaphase .
	manualset3
253217	5	425775	7	NULL	NULL	0	NULL	pathology	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Cooling causes a sharp rise of the pathological mitosis , represented mainly by the forms of pathology connected with the disorganization of the mitotic apparatus , such as C-mitosis and dispersion of chromosomes in the metaphase .
	manualset3
253218	6	425775	7	NULL	NULL	0	NULL	disorganization 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cooling causes a sharp rise of the pathological mitosis , represented mainly by the forms of pathology connected with the disorganization of the mitotic apparatus , such as C-mitosis and dispersion of chromosomes in the metaphase .
	manualset3
253219	7	425775	7	NULL	NULL	0	NULL	 mitotic apparatus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Cooling causes a sharp rise of the pathological mitosis , represented mainly by the forms of pathology connected with the disorganization of the mitotic apparatus , such as C-mitosis and dispersion of chromosomes in the metaphase .
	manualset3
253220	8	425775	7	NULL	NULL	0	NULL	C-mitosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cooling causes a sharp rise of the pathological mitosis , represented mainly by the forms of pathology connected with the disorganization of the mitotic apparatus , such as C-mitosis and dispersion of chromosomes in the metaphase .
	manualset3
253221	9	425775	7	NULL	NULL	0	NULL	dispersion 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cooling causes a sharp rise of the pathological mitosis , represented mainly by the forms of pathology connected with the disorganization of the mitotic apparatus , such as C-mitosis and dispersion of chromosomes in the metaphase .
	manualset3
253222	10	425775	7	NULL	NULL	0	NULL	chromosomes	Chromosome												NULL		0	NULL	NULL	NULL	NULL	NULL	Cooling causes a sharp rise of the pathological mitosis , represented mainly by the forms of pathology connected with the disorganization of the mitotic apparatus , such as C-mitosis and dispersion of chromosomes in the metaphase .
	manualset3
253223	11	425775	7	NULL	NULL	0	NULL	 metaphase 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cooling causes a sharp rise of the pathological mitosis , represented mainly by the forms of pathology connected with the disorganization of the mitotic apparatus , such as C-mitosis and dispersion of chromosomes in the metaphase .
	manualset3
253224	1	425776	7	NULL	NULL	0	NULL	Cooling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Cooling was found to reduce the response amplitude , decrease the time course , and increase the latency .
	manualset3
253225	2	425776	7	NULL	NULL	0	NULL	response amplitude	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Cooling was found to reduce the response amplitude , decrease the time course , and increase the latency .
	manualset3
253226	3	425776	7	NULL	NULL	0	NULL	decrease	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Cooling was found to reduce the response amplitude , decrease the time course , and increase the latency .
	manualset3
253227	4	425776	7	NULL	NULL	0	NULL	time course	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Cooling was found to reduce the response amplitude , decrease the time course , and increase the latency .
	manualset3
253228	7	425776	7	NULL	NULL	NULL	NULL	latency	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cooling was found to reduce the response amplitude , decrease the time course , and increase the latency .
	manualset3
253229	6	425776	7	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Cooling was found to reduce the response amplitude , decrease the time course , and increase the latency .
	manualset3
253230	1	425777	7	NULL	NULL	0	NULL	Cooperative extraction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Cooperative extraction of membrane nanotubes by molecular motors .
	manualset3
253231	2	425777	7	NULL	NULL	0	NULL	membrane nanotubes	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Cooperative extraction of membrane nanotubes by molecular motors .
	manualset3
253232	3	425777	7	NULL	NULL	0	NULL	molecular motors	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Cooperative extraction of membrane nanotubes by molecular motors .
	manualset3
253233	1	425778	7	NULL	NULL	0	NULL	Cooperative interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cooperative interaction between interferon ( IFN ) stimulus response element and kappa B sequence motifs controls IFN gamma - and lipopolysaccharide-stimulated transcription from the murine IP-10 promoter .
	manualset3
253234	2	425778	7	NULL	NULL	0	NULL	interferon ( IFN ) stimulus response element	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Cooperative interaction between interferon ( IFN ) stimulus response element and kappa B sequence motifs controls IFN gamma - and lipopolysaccharide-stimulated transcription from the murine IP-10 promoter .
	manualset3
253235	3	425778	7	NULL	NULL	0	NULL	 kappa B sequence motifs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Cooperative interaction between interferon ( IFN ) stimulus response element and kappa B sequence motifs controls IFN gamma - and lipopolysaccharide-stimulated transcription from the murine IP-10 promoter .
	manualset3
253236	4	425778	7	NULL	NULL	NULL	NULL	IFN gamma-stimulated transcription	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cooperative interaction between interferon ( IFN ) stimulus response element and kappa B sequence motifs controls IFN gamma - and lipopolysaccharide-stimulated transcription from the murine IP-10 promoter .
	manualset3
253237	5	425778	7	NULL	NULL	0	NULL	murine IP-10 promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Cooperative interaction between interferon ( IFN ) stimulus response element and kappa B sequence motifs controls IFN gamma - and lipopolysaccharide-stimulated transcription from the murine IP-10 promoter .
	manualset3
256775	6	425778	7	NULL	NULL	NULL	NULL	lipopolysaccharide-stimulated transcription	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cooperative interaction between interferon ( IFN ) stimulus response element and kappa B sequence motifs controls IFN gamma - and lipopolysaccharide-stimulated transcription from the murine IP-10 promoter .
	manualset3
253238	1	425779	7	NULL	NULL	0	NULL	Coordination 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Coordination of DNA synthesis and replicative unwinding by the S-phase checkpoint pathways .
	manualset3
253239	2	425779	7	NULL	NULL	0	NULL	DNA synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Coordination of DNA synthesis and replicative unwinding by the S-phase checkpoint pathways .
	manualset3
253240	3	425779	7	NULL	NULL	0	NULL	replicative unwinding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Coordination of DNA synthesis and replicative unwinding by the S-phase checkpoint pathways .
	manualset3
253241	4	425779	7	NULL	NULL	0	NULL	S-phase checkpoint pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Coordination of DNA synthesis and replicative unwinding by the S-phase checkpoint pathways .
	manualset3
253242	1	425780	7	NULL	NULL	0	NULL	Copeptin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Copeptin was highest on admission ( 40.0 + / - 72.3 pmol/l ) , stabilized on day 3 and 7 ( 21.2 + / - 18.3 resp .
	manualset3
253243	2	425780	7	NULL	NULL	NULL	NULL	admission	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Copeptin was highest on admission ( 40.0 + / - 72.3 pmol/l ) , stabilized on day 3 and 7 ( 21.2 + / - 18.3 resp .
	manualset3
253244	3	425780	7	NULL	NULL	NULL	NULL	40.0 + / - 72.3 pmol/l 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Copeptin was highest on admission ( 40.0 + / - 72.3 pmol/l ) , stabilized on day 3 and 7 ( 21.2 + / - 18.3 resp .
	manualset3
253245	4	425780	7	NULL	NULL	0	NULL	day 3 	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Copeptin was highest on admission ( 40.0 + / - 72.3 pmol/l ) , stabilized on day 3 and 7 ( 21.2 + / - 18.3 resp .
	manualset3
253246	5	425780	7	NULL	NULL	0	NULL	day 7	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Copeptin was highest on admission ( 40.0 + / - 72.3 pmol/l ) , stabilized on day 3 and 7 ( 21.2 + / - 18.3 resp .
	manualset3
253247	6	425780	7	NULL	NULL	0	NULL	21.2 + / - 18.3	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Copeptin was highest on admission ( 40.0 + / - 72.3 pmol/l ) , stabilized on day 3 and 7 ( 21.2 + / - 18.3 resp .
	manualset3
253248	1	425781	7	NULL	NULL	0	NULL	Copper-binding protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Copper-binding protein in liver cells .
	manualset3
253249	2	425781	7	NULL	NULL	0	NULL	liver cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Copper-binding protein in liver cells .
	manualset3
253250	1	425782	7	NULL	NULL	NULL	NULL	Copper ( II ) - catalyzed highly enantioselective addition	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Copper ( II ) - catalyzed highly enantioselective addition of enamides to imines : the use of enamides as nucleophiles in asymmetric catalysis .
	manualset3
253252	3	425782	7	NULL	NULL	0	NULL	enamides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Copper ( II ) - catalyzed highly enantioselective addition of enamides to imines : the use of enamides as nucleophiles in asymmetric catalysis .
	manualset3
253253	4	425782	7	NULL	NULL	0	NULL	imines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Copper ( II ) - catalyzed highly enantioselective addition of enamides to imines : the use of enamides as nucleophiles in asymmetric catalysis .
	manualset3
253254	5	425782	7	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Copper ( II ) - catalyzed highly enantioselective addition of enamides to imines : the use of enamides as nucleophiles in asymmetric catalysis .
	manualset3
253255	6	425782	7	NULL	NULL	0	NULL	enamides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Copper ( II ) - catalyzed highly enantioselective addition of enamides to imines : the use of enamides as nucleophiles in asymmetric catalysis .
	manualset3
253256	7	425782	7	NULL	NULL	0	NULL	nucleophiles 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Copper ( II ) - catalyzed highly enantioselective addition of enamides to imines : the use of enamides as nucleophiles in asymmetric catalysis .
	manualset3
253257	8	425782	7	NULL	NULL	0	NULL	 asymmetric catalysis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Copper ( II ) - catalyzed highly enantioselective addition of enamides to imines : the use of enamides as nucleophiles in asymmetric catalysis .
	manualset3
253258	1	425783	7	NULL	NULL	0	NULL	Copulation-illness associations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Copulation-illness associations in male rats : lithium chloride dose and delay manipulations .
	manualset3
253259	2	425783	7	NULL	NULL	0	NULL	male rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Copulation-illness associations in male rats : lithium chloride dose and delay manipulations .
	manualset3
253260	3	425783	7	NULL	NULL	0	NULL	lithium chloride dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Copulation-illness associations in male rats : lithium chloride dose and delay manipulations .
	manualset3
253261	4	425783	7	NULL	NULL	0	NULL	delay manipulations 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Copulation-illness associations in male rats : lithium chloride dose and delay manipulations .
	manualset3
253262	1	425784	7	NULL	NULL	0	NULL	Cord blood MSCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Cord blood MSCs may be involved in innate immune systems as the neonatal defense system against the earliest encountered pathogens .
	manualset3
253263	2	425784	7	NULL	NULL	0	NULL	innate immune systems	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cord blood MSCs may be involved in innate immune systems as the neonatal defense system against the earliest encountered pathogens .
	manualset3
253264	3	425784	7	NULL	NULL	0	NULL	neonatal defense system	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cord blood MSCs may be involved in innate immune systems as the neonatal defense system against the earliest encountered pathogens .
	manualset3
253265	4	425784	7	NULL	NULL	NULL	NULL	earliest encountered pathogens	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cord blood MSCs may be involved in innate immune systems as the neonatal defense system against the earliest encountered pathogens .
	manualset3
253266	1	425785	7	NULL	NULL	0	NULL	Cord compression 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Cord compression developed in 3 of 4 dogs in the 0.58 mg/kg IV Early group ; 2 of 3 dogs in the IT + IV Early group ; and 0 of 4 dogs in the 1.57 mg/kg IV Early group by 12-18months of age .
	manualset3
253267	2	425785	7	NULL	NULL	0	NULL	3 of 4 dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Cord compression developed in 3 of 4 dogs in the 0.58 mg/kg IV Early group ; 2 of 3 dogs in the IT + IV Early group ; and 0 of 4 dogs in the 1.57 mg/kg IV Early group by 12-18months of age .
	manualset3
253268	3	425785	7	NULL	NULL	0	NULL	0.58 mg/kg IV Early group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Cord compression developed in 3 of 4 dogs in the 0.58 mg/kg IV Early group ; 2 of 3 dogs in the IT + IV Early group ; and 0 of 4 dogs in the 1.57 mg/kg IV Early group by 12-18months of age .
	manualset3
253269	4	425785	7	NULL	NULL	0	NULL	2 of 3 dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Cord compression developed in 3 of 4 dogs in the 0.58 mg/kg IV Early group ; 2 of 3 dogs in the IT + IV Early group ; and 0 of 4 dogs in the 1.57 mg/kg IV Early group by 12-18months of age .
	manualset3
253270	5	425785	7	NULL	NULL	0	NULL	IT + IV Early group 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Cord compression developed in 3 of 4 dogs in the 0.58 mg/kg IV Early group ; 2 of 3 dogs in the IT + IV Early group ; and 0 of 4 dogs in the 1.57 mg/kg IV Early group by 12-18months of age .
	manualset3
253271	6	425785	7	NULL	NULL	0	NULL	0 of 4 dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Cord compression developed in 3 of 4 dogs in the 0.58 mg/kg IV Early group ; 2 of 3 dogs in the IT + IV Early group ; and 0 of 4 dogs in the 1.57 mg/kg IV Early group by 12-18months of age .
	manualset3
253272	7	425785	7	NULL	NULL	0	NULL	1.57 mg/kg IV Early group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Cord compression developed in 3 of 4 dogs in the 0.58 mg/kg IV Early group ; 2 of 3 dogs in the IT + IV Early group ; and 0 of 4 dogs in the 1.57 mg/kg IV Early group by 12-18months of age .
	manualset3
253273	8	425785	7	NULL	NULL	0	NULL	 12-18months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Cord compression developed in 3 of 4 dogs in the 0.58 mg/kg IV Early group ; 2 of 3 dogs in the IT + IV Early group ; and 0 of 4 dogs in the 1.57 mg/kg IV Early group by 12-18months of age .
	manualset3
253274	9	425785	7	NULL	NULL	0	NULL	age	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cord compression developed in 3 of 4 dogs in the 0.58 mg/kg IV Early group ; 2 of 3 dogs in the IT + IV Early group ; and 0 of 4 dogs in the 1.57 mg/kg IV Early group by 12-18months of age .
	manualset3
253275	1	425786	7	NULL	NULL	0	NULL	Cord tethering	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Cord tethering induced a reduction of rSCBF in the distal spinal cord close to the tethering ( L3 ) by 32 % of the normal flow 2 weeks after tethering and by 67 % 10 weeks after tethering .
	manualset3
253276	2	425786	7	NULL	NULL	0	NULL	reduction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cord tethering induced a reduction of rSCBF in the distal spinal cord close to the tethering ( L3 ) by 32 % of the normal flow 2 weeks after tethering and by 67 % 10 weeks after tethering .
	manualset3
253277	3	425786	7	NULL	NULL	0	NULL	rSCBF	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cord tethering induced a reduction of rSCBF in the distal spinal cord close to the tethering ( L3 ) by 32 % of the normal flow 2 weeks after tethering and by 67 % 10 weeks after tethering .
	manualset3
253278	4	425786	7	NULL	NULL	0	NULL	 distal spinal cord	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Cord tethering induced a reduction of rSCBF in the distal spinal cord close to the tethering ( L3 ) by 32 % of the normal flow 2 weeks after tethering and by 67 % 10 weeks after tethering .
	manualset3
253279	5	425786	7	NULL	NULL	NULL	NULL	tethering ( L3 )	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cord tethering induced a reduction of rSCBF in the distal spinal cord close to the tethering ( L3 ) by 32 % of the normal flow 2 weeks after tethering and by 67 % 10 weeks after tethering .
	manualset3
253280	6	425786	7	NULL	NULL	0	NULL	32 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Cord tethering induced a reduction of rSCBF in the distal spinal cord close to the tethering ( L3 ) by 32 % of the normal flow 2 weeks after tethering and by 67 % 10 weeks after tethering .
	manualset3
253281	7	425786	7	NULL	NULL	0	NULL	normal flow 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Cord tethering induced a reduction of rSCBF in the distal spinal cord close to the tethering ( L3 ) by 32 % of the normal flow 2 weeks after tethering and by 67 % 10 weeks after tethering .
	manualset3
253282	8	425786	7	NULL	NULL	0	NULL	2 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Cord tethering induced a reduction of rSCBF in the distal spinal cord close to the tethering ( L3 ) by 32 % of the normal flow 2 weeks after tethering and by 67 % 10 weeks after tethering .
	manualset3
253283	9	425786	7	NULL	NULL	NULL	NULL	tethering	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cord tethering induced a reduction of rSCBF in the distal spinal cord close to the tethering ( L3 ) by 32 % of the normal flow 2 weeks after tethering and by 67 % 10 weeks after tethering .
	manualset3
253284	10	425786	7	NULL	NULL	0	NULL	 67 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Cord tethering induced a reduction of rSCBF in the distal spinal cord close to the tethering ( L3 ) by 32 % of the normal flow 2 weeks after tethering and by 67 % 10 weeks after tethering .
	manualset3
253285	11	425786	7	NULL	NULL	0	NULL	10 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Cord tethering induced a reduction of rSCBF in the distal spinal cord close to the tethering ( L3 ) by 32 % of the normal flow 2 weeks after tethering and by 67 % 10 weeks after tethering .
	manualset3
253286	12	425786	7	NULL	NULL	0	NULL	 tethering	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Cord tethering induced a reduction of rSCBF in the distal spinal cord close to the tethering ( L3 ) by 32 % of the normal flow 2 weeks after tethering and by 67 % 10 weeks after tethering .
	manualset3
253287	1	425787	7	NULL	NULL	NULL	NULL	MECHANISM	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( MECHANISM OF MUSCULAR ACTION OF ETHANOL ON THE ISOLATED RAT GASTRO-PYLORIC PREPARATION ) .
	manualset3
253288	2	425787	7	NULL	NULL	0	NULL	MUSCULAR ACTION	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( MECHANISM OF MUSCULAR ACTION OF ETHANOL ON THE ISOLATED RAT GASTRO-PYLORIC PREPARATION ) .
	manualset3
253289	3	425787	7	NULL	NULL	0	NULL	ETHANOL	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( MECHANISM OF MUSCULAR ACTION OF ETHANOL ON THE ISOLATED RAT GASTRO-PYLORIC PREPARATION ) .
	manualset3
253290	4	425787	7	NULL	NULL	0	NULL	ISOLATED RAT GASTRO-PYLORIC PREPARATION	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	( MECHANISM OF MUSCULAR ACTION OF ETHANOL ON THE ISOLATED RAT GASTRO-PYLORIC PREPARATION ) .
	manualset3
253291	1	425788	7	NULL	NULL	0	NULL	Coronary angioplasty	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Coronary angioplasty was performed with either direct stenting or after balloon predilatation .
	manualset3
253292	2	425788	7	NULL	NULL	0	NULL	direct stenting	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Coronary angioplasty was performed with either direct stenting or after balloon predilatation .
	manualset3
253293	3	425788	7	NULL	NULL	0	NULL	balloon predilatation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Coronary angioplasty was performed with either direct stenting or after balloon predilatation .
	manualset3
253294	1	425789	7	NULL	NULL	0	NULL	Coronary arterial diameter	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Coronary arterial diameter during ventricular pacing significantly increased compared to that during both sinus rhythm and atrial pacing .
	manualset3
253295	2	425789	7	NULL	NULL	0	NULL	ventricular pacing	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Coronary arterial diameter during ventricular pacing significantly increased compared to that during both sinus rhythm and atrial pacing .
	manualset3
253296	3	425789	7	NULL	NULL	0	NULL	sinus rhythm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Coronary arterial diameter during ventricular pacing significantly increased compared to that during both sinus rhythm and atrial pacing .
	manualset3
253297	4	425789	7	NULL	NULL	0	NULL	atrial pacing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Coronary arterial diameter during ventricular pacing significantly increased compared to that during both sinus rhythm and atrial pacing .
	manualset3
253298	1	425790	7	NULL	NULL	0	NULL	Coronary blood flow	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Coronary blood flow and flow reserve in aortic stenosis : effect of aortic valve therapy .
	manualset3
253299	2	425790	7	NULL	NULL	0	NULL	 flow reserve	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Coronary blood flow and flow reserve in aortic stenosis : effect of aortic valve therapy .
	manualset3
253300	3	425790	7	NULL	NULL	0	NULL	aortic stenosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Coronary blood flow and flow reserve in aortic stenosis : effect of aortic valve therapy .
	manualset3
253301	4	425790	7	NULL	NULL	0	NULL	 effect 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Coronary blood flow and flow reserve in aortic stenosis : effect of aortic valve therapy .
	manualset3
253302	5	425790	7	NULL	NULL	0	NULL	aortic valve therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Coronary blood flow and flow reserve in aortic stenosis : effect of aortic valve therapy .
	manualset3
253303	1	425791	7	NULL	NULL	0	NULL	Coronary heart disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Coronary heart disease is the leading cause of death among the elderly ( ) 65 years ) and the very elderly ( ) 85 years ) .
	manualset3
253304	2	425791	7	NULL	NULL	0	NULL	leading cause	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Coronary heart disease is the leading cause of death among the elderly ( ) 65 years ) and the very elderly ( ) 85 years ) .
	manualset3
253305	3	425791	7	NULL	NULL	0	NULL	 death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Coronary heart disease is the leading cause of death among the elderly ( ) 65 years ) and the very elderly ( ) 85 years ) .
	manualset3
253306	4	425791	7	NULL	NULL	0	NULL	65 years 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Coronary heart disease is the leading cause of death among the elderly ( ) 65 years ) and the very elderly ( ) 85 years ) .
	manualset3
253307	5	425791	7	NULL	NULL	0	NULL	85 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Coronary heart disease is the leading cause of death among the elderly ( ) 65 years ) and the very elderly ( ) 85 years ) .
	manualset3
253308	1	425792	7	NULL	NULL	0	NULL	Corps ronds	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Corps ronds occurred at the basal aspect of spinous layer , while grains were abundant in the bulla and in the granular layer of the peripheral epidermis .
	manualset3
253309	2	425792	7	NULL	NULL	0	NULL	basal aspect 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Corps ronds occurred at the basal aspect of spinous layer , while grains were abundant in the bulla and in the granular layer of the peripheral epidermis .
	manualset3
253310	3	425792	7	NULL	NULL	0	NULL	spinous layer	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Corps ronds occurred at the basal aspect of spinous layer , while grains were abundant in the bulla and in the granular layer of the peripheral epidermis .
	manualset3
253311	4	425792	7	NULL	NULL	0	NULL	grains	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Corps ronds occurred at the basal aspect of spinous layer , while grains were abundant in the bulla and in the granular layer of the peripheral epidermis .
	manualset3
253312	5	425792	7	NULL	NULL	0	NULL	bulla	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Corps ronds occurred at the basal aspect of spinous layer , while grains were abundant in the bulla and in the granular layer of the peripheral epidermis .
	manualset3
253313	6	425792	7	NULL	NULL	0	NULL	granular layer	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Corps ronds occurred at the basal aspect of spinous layer , while grains were abundant in the bulla and in the granular layer of the peripheral epidermis .
	manualset3
253314	7	425792	7	NULL	NULL	0	NULL	peripheral epidermis	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Corps ronds occurred at the basal aspect of spinous layer , while grains were abundant in the bulla and in the granular layer of the peripheral epidermis .
	manualset3
253315	1	425793	7	NULL	NULL	0	NULL	Correction 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Correction to the interfacial tension by curvature radius : differences between droplets and bubbles .
	manualset3
253316	2	425793	7	NULL	NULL	0	NULL	 interfacial tension	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Correction to the interfacial tension by curvature radius : differences between droplets and bubbles .
	manualset3
253317	3	425793	7	NULL	NULL	0	NULL	curvature radius	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Correction to the interfacial tension by curvature radius : differences between droplets and bubbles .
	manualset3
253318	4	425793	7	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Correction to the interfacial tension by curvature radius : differences between droplets and bubbles .
	manualset3
253319	5	425793	7	NULL	NULL	0	NULL	droplets	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Correction to the interfacial tension by curvature radius : differences between droplets and bubbles .
	manualset3
253320	6	425793	7	NULL	NULL	0	NULL	bubbles	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Correction to the interfacial tension by curvature radius : differences between droplets and bubbles .
	manualset3
253321	1	425794	7	NULL	NULL	0	NULL	Correlated components	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlated components of ongoing EEG point to emotionally laden attention - a possible marker of engagement ?
	manualset3
253322	2	425794	7	NULL	NULL	0	NULL	ongoing EEG	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlated components of ongoing EEG point to emotionally laden attention - a possible marker of engagement ?
	manualset3
253323	3	425794	7	NULL	NULL	0	NULL	emotionally laden attention	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlated components of ongoing EEG point to emotionally laden attention - a possible marker of engagement ?
	manualset3
253324	4	425794	7	NULL	NULL	NULL	NULL	marker 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Correlated components of ongoing EEG point to emotionally laden attention - a possible marker of engagement ?
	manualset3
257001	5	425794	7	NULL	NULL	NULL	NULL	 engagement	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Correlated components of ongoing EEG point to emotionally laden attention - a possible marker of engagement ?
	manualset3
253325	1	425795	7	NULL	NULL	0	NULL	Correlation 's	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation 's : significant negative correlation was found between ST and D4/P4 for creatinine ( r = -0.45 , p & lt ; 0.005 ) and significant positive correlation between ST and D4/DO for glucose ( r = 0.48 , p = 0.003 ) .
	manualset3
253326	2	425795	7	NULL	NULL	0	NULL	negative correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation 's : significant negative correlation was found between ST and D4/P4 for creatinine ( r = -0.45 , p & lt ; 0.005 ) and significant positive correlation between ST and D4/DO for glucose ( r = 0.48 , p = 0.003 ) .
	manualset3
253327	3	425795	7	NULL	NULL	0	NULL	ST	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation 's : significant negative correlation was found between ST and D4/P4 for creatinine ( r = -0.45 , p & lt ; 0.005 ) and significant positive correlation between ST and D4/DO for glucose ( r = 0.48 , p = 0.003 ) .
	manualset3
253328	4	425795	7	NULL	NULL	0	NULL	D4/P4	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation 's : significant negative correlation was found between ST and D4/P4 for creatinine ( r = -0.45 , p & lt ; 0.005 ) and significant positive correlation between ST and D4/DO for glucose ( r = 0.48 , p = 0.003 ) .
	manualset3
253329	5	425795	7	NULL	NULL	0	NULL	creatinine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation 's : significant negative correlation was found between ST and D4/P4 for creatinine ( r = -0.45 , p & lt ; 0.005 ) and significant positive correlation between ST and D4/DO for glucose ( r = 0.48 , p = 0.003 ) .
	manualset3
253330	6	425795	7	NULL	NULL	0	NULL	r = -0.45	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation 's : significant negative correlation was found between ST and D4/P4 for creatinine ( r = -0.45 , p & lt ; 0.005 ) and significant positive correlation between ST and D4/DO for glucose ( r = 0.48 , p = 0.003 ) .
	manualset3
253331	7	425795	7	NULL	NULL	0	NULL	p & lt ; 0.005	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation 's : significant negative correlation was found between ST and D4/P4 for creatinine ( r = -0.45 , p & lt ; 0.005 ) and significant positive correlation between ST and D4/DO for glucose ( r = 0.48 , p = 0.003 ) .
	manualset3
253332	8	425795	7	NULL	NULL	0	NULL	positive correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation 's : significant negative correlation was found between ST and D4/P4 for creatinine ( r = -0.45 , p & lt ; 0.005 ) and significant positive correlation between ST and D4/DO for glucose ( r = 0.48 , p = 0.003 ) .
	manualset3
253333	9	425795	7	NULL	NULL	0	NULL	ST	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation 's : significant negative correlation was found between ST and D4/P4 for creatinine ( r = -0.45 , p & lt ; 0.005 ) and significant positive correlation between ST and D4/DO for glucose ( r = 0.48 , p = 0.003 ) .
	manualset3
253334	10	425795	7	NULL	NULL	0	NULL	D4/DO	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation 's : significant negative correlation was found between ST and D4/P4 for creatinine ( r = -0.45 , p & lt ; 0.005 ) and significant positive correlation between ST and D4/DO for glucose ( r = 0.48 , p = 0.003 ) .
	manualset3
253335	11	425795	7	NULL	NULL	0	NULL	glucose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation 's : significant negative correlation was found between ST and D4/P4 for creatinine ( r = -0.45 , p & lt ; 0.005 ) and significant positive correlation between ST and D4/DO for glucose ( r = 0.48 , p = 0.003 ) .
	manualset3
253336	12	425795	7	NULL	NULL	0	NULL	r = 0.48	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation 's : significant negative correlation was found between ST and D4/P4 for creatinine ( r = -0.45 , p & lt ; 0.005 ) and significant positive correlation between ST and D4/DO for glucose ( r = 0.48 , p = 0.003 ) .
	manualset3
253337	13	425795	7	NULL	NULL	0	NULL	p = 0.003	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation 's : significant negative correlation was found between ST and D4/P4 for creatinine ( r = -0.45 , p & lt ; 0.005 ) and significant positive correlation between ST and D4/DO for glucose ( r = 0.48 , p = 0.003 ) .
	manualset3
253338	1	425796	7	NULL	NULL	0	NULL	Correlation analyses	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation analyses of root and leaf Zn and Fe contents suggested that Zn may interfere with the translocation of Fe ; however , Zn toxicity was not associated with a diminished leaf Fe content .
	manualset3
253339	2	425796	7	NULL	NULL	0	NULL	 root 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation analyses of root and leaf Zn and Fe contents suggested that Zn may interfere with the translocation of Fe ; however , Zn toxicity was not associated with a diminished leaf Fe content .
	manualset3
253340	3	425796	7	NULL	NULL	0	NULL	 leaf	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation analyses of root and leaf Zn and Fe contents suggested that Zn may interfere with the translocation of Fe ; however , Zn toxicity was not associated with a diminished leaf Fe content .
	manualset3
253341	4	425796	7	NULL	NULL	0	NULL	Zn contents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation analyses of root and leaf Zn and Fe contents suggested that Zn may interfere with the translocation of Fe ; however , Zn toxicity was not associated with a diminished leaf Fe content .
	manualset3
253342	5	425796	7	NULL	NULL	0	NULL	Fe contents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation analyses of root and leaf Zn and Fe contents suggested that Zn may interfere with the translocation of Fe ; however , Zn toxicity was not associated with a diminished leaf Fe content .
	manualset3
253343	6	425796	7	NULL	NULL	0	NULL	Zn	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation analyses of root and leaf Zn and Fe contents suggested that Zn may interfere with the translocation of Fe ; however , Zn toxicity was not associated with a diminished leaf Fe content .
	manualset3
253344	7	425796	7	NULL	NULL	0	NULL	translocation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation analyses of root and leaf Zn and Fe contents suggested that Zn may interfere with the translocation of Fe ; however , Zn toxicity was not associated with a diminished leaf Fe content .
	manualset3
253345	8	425796	7	NULL	NULL	0	NULL	Fe	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation analyses of root and leaf Zn and Fe contents suggested that Zn may interfere with the translocation of Fe ; however , Zn toxicity was not associated with a diminished leaf Fe content .
	manualset3
253346	9	425796	7	NULL	NULL	0	NULL	Zn toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation analyses of root and leaf Zn and Fe contents suggested that Zn may interfere with the translocation of Fe ; however , Zn toxicity was not associated with a diminished leaf Fe content .
	manualset3
253347	10	425796	7	NULL	NULL	NULL	NULL	leaf Fe content	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Correlation analyses of root and leaf Zn and Fe contents suggested that Zn may interfere with the translocation of Fe ; however , Zn toxicity was not associated with a diminished leaf Fe content .
	manualset3
253348	1	425797	7	NULL	NULL	0	NULL	Correlation analyses	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation analyses were performed to investigate the relation between patient satisfaction and the 2 different aspects of the outcome scales : postoperative scores evaluated at latest follow-ups and preoperative to postoperative changes .
	manualset3
253349	2	425797	7	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation analyses were performed to investigate the relation between patient satisfaction and the 2 different aspects of the outcome scales : postoperative scores evaluated at latest follow-ups and preoperative to postoperative changes .
	manualset3
253350	3	425797	7	NULL	NULL	0	NULL	 patient satisfaction	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation analyses were performed to investigate the relation between patient satisfaction and the 2 different aspects of the outcome scales : postoperative scores evaluated at latest follow-ups and preoperative to postoperative changes .
	manualset3
253351	4	425797	7	NULL	NULL	0	NULL	2 different aspects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation analyses were performed to investigate the relation between patient satisfaction and the 2 different aspects of the outcome scales : postoperative scores evaluated at latest follow-ups and preoperative to postoperative changes .
	manualset3
253352	5	425797	7	NULL	NULL	0	NULL	outcome scales	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation analyses were performed to investigate the relation between patient satisfaction and the 2 different aspects of the outcome scales : postoperative scores evaluated at latest follow-ups and preoperative to postoperative changes .
	manualset3
253353	6	425797	7	NULL	NULL	0	NULL	postoperative scores	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation analyses were performed to investigate the relation between patient satisfaction and the 2 different aspects of the outcome scales : postoperative scores evaluated at latest follow-ups and preoperative to postoperative changes .
	manualset3
253354	7	425797	7	NULL	NULL	0	NULL	follow-ups	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation analyses were performed to investigate the relation between patient satisfaction and the 2 different aspects of the outcome scales : postoperative scores evaluated at latest follow-ups and preoperative to postoperative changes .
	manualset3
253355	8	425797	7	NULL	NULL	0	NULL	preoperative changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation analyses were performed to investigate the relation between patient satisfaction and the 2 different aspects of the outcome scales : postoperative scores evaluated at latest follow-ups and preoperative to postoperative changes .
	manualset3
253356	9	425797	7	NULL	NULL	0	NULL	 postoperative changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation analyses were performed to investigate the relation between patient satisfaction and the 2 different aspects of the outcome scales : postoperative scores evaluated at latest follow-ups and preoperative to postoperative changes .
	manualset3
253357	1	425798	7	NULL	NULL	0	NULL	Correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between anthropometric parameters and abdominal fat volumes assessed by a magnetic resonance imaging method in patients with diabetes .
	manualset3
253358	2	425798	7	NULL	NULL	0	NULL	anthropometric parameters 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between anthropometric parameters and abdominal fat volumes assessed by a magnetic resonance imaging method in patients with diabetes .
	manualset3
253359	3	425798	7	NULL	NULL	0	NULL	abdominal fat volumes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between anthropometric parameters and abdominal fat volumes assessed by a magnetic resonance imaging method in patients with diabetes .
	manualset3
253360	4	425798	7	NULL	NULL	0	NULL	 magnetic resonance imaging method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between anthropometric parameters and abdominal fat volumes assessed by a magnetic resonance imaging method in patients with diabetes .
	manualset3
253361	5	425798	7	NULL	NULL	0	NULL	 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between anthropometric parameters and abdominal fat volumes assessed by a magnetic resonance imaging method in patients with diabetes .
	manualset3
253362	6	425798	7	NULL	NULL	0	NULL	diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between anthropometric parameters and abdominal fat volumes assessed by a magnetic resonance imaging method in patients with diabetes .
	manualset3
253363	1	425799	7	NULL	NULL	0	NULL	Correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between light - and electron-microscopic appearance has been demonstrated .
	manualset3
253364	2	425799	7	NULL	NULL	0	NULL	light -appearance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between light - and electron-microscopic appearance has been demonstrated .
	manualset3
253365	3	425799	7	NULL	NULL	0	NULL	electron-microscopic appearance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between light - and electron-microscopic appearance has been demonstrated .
	manualset3
253366	1	425800	7	NULL	NULL	0	NULL	Correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between postsialographical changes of salivary isoamylase levels in serum and histopathological findings in sublingual glands in patients with Sjgren 's syndrome .
	manualset3
253367	2	425800	7	NULL	NULL	0	NULL	postsialographical changes 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between postsialographical changes of salivary isoamylase levels in serum and histopathological findings in sublingual glands in patients with Sjgren 's syndrome .
	manualset3
253368	3	425800	7	NULL	NULL	0	NULL	salivary isoamylase levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between postsialographical changes of salivary isoamylase levels in serum and histopathological findings in sublingual glands in patients with Sjgren 's syndrome .
	manualset3
253369	4	425800	7	NULL	NULL	0	NULL	serum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between postsialographical changes of salivary isoamylase levels in serum and histopathological findings in sublingual glands in patients with Sjgren 's syndrome .
	manualset3
253370	5	425800	7	NULL	NULL	0	NULL	histopathological findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between postsialographical changes of salivary isoamylase levels in serum and histopathological findings in sublingual glands in patients with Sjgren 's syndrome .
	manualset3
253371	6	425800	7	NULL	NULL	0	NULL	sublingual glands	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between postsialographical changes of salivary isoamylase levels in serum and histopathological findings in sublingual glands in patients with Sjgren 's syndrome .
	manualset3
253372	7	425800	7	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between postsialographical changes of salivary isoamylase levels in serum and histopathological findings in sublingual glands in patients with Sjgren 's syndrome .
	manualset3
253373	8	425800	7	NULL	NULL	0	NULL	Sjgren 's syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between postsialographical changes of salivary isoamylase levels in serum and histopathological findings in sublingual glands in patients with Sjgren 's syndrome .
	manualset3
253374	1	425801	7	NULL	NULL	0	NULL	MRSA infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( MRSA infection in emergency departments ) .
	manualset3
253375	2	425801	7	NULL	NULL	0	NULL	emergency departments 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( MRSA infection in emergency departments ) .
	manualset3
253376	1	425802	7	NULL	NULL	0	NULL	Correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between telomerase expression and terminal restriction fragment length ratio in non-small cell lung cancer -- an adjusted measurement and its clinical significance .
	manualset3
253377	2	425802	7	NULL	NULL	0	NULL	telomerase expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between telomerase expression and terminal restriction fragment length ratio in non-small cell lung cancer -- an adjusted measurement and its clinical significance .
	manualset3
253378	3	425802	7	NULL	NULL	0	NULL	terminal restriction fragment length ratio	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between telomerase expression and terminal restriction fragment length ratio in non-small cell lung cancer -- an adjusted measurement and its clinical significance .
	manualset3
253379	4	425802	7	NULL	NULL	0	NULL	non-small cell lung cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between telomerase expression and terminal restriction fragment length ratio in non-small cell lung cancer -- an adjusted measurement and its clinical significance .
	manualset3
253380	5	425802	7	NULL	NULL	0	NULL	measurement	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between telomerase expression and terminal restriction fragment length ratio in non-small cell lung cancer -- an adjusted measurement and its clinical significance .
	manualset3
253381	6	425802	7	NULL	NULL	0	NULL	clinical significance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation between telomerase expression and terminal restriction fragment length ratio in non-small cell lung cancer -- an adjusted measurement and its clinical significance .
	manualset3
253382	1	425803	7	NULL	NULL	0	NULL	Correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation of 18F-FLT and 18F-FDG uptake on PET with Ki-67 immunohistochemistry in non-small cell lung cancer .
	manualset3
253383	2	425803	7	NULL	NULL	NULL	NULL	18F-FLT uptake	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Correlation of 18F-FLT and 18F-FDG uptake on PET with Ki-67 immunohistochemistry in non-small cell lung cancer .
	manualset3
253384	3	425803	7	NULL	NULL	0	NULL	18F-FDG uptake	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation of 18F-FLT and 18F-FDG uptake on PET with Ki-67 immunohistochemistry in non-small cell lung cancer .
	manualset3
253385	4	425803	7	NULL	NULL	0	NULL	PET	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation of 18F-FLT and 18F-FDG uptake on PET with Ki-67 immunohistochemistry in non-small cell lung cancer .
	manualset3
253386	5	425803	7	NULL	NULL	0	NULL	Ki-67 immunohistochemistry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation of 18F-FLT and 18F-FDG uptake on PET with Ki-67 immunohistochemistry in non-small cell lung cancer .
	manualset3
253387	6	425803	7	NULL	NULL	0	NULL	non-small cell lung cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation of 18F-FLT and 18F-FDG uptake on PET with Ki-67 immunohistochemistry in non-small cell lung cancer .
	manualset3
253388	1	425804	7	NULL	NULL	0	NULL	Correlation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation of contractile function and passive properties of rabbit urinary bladder subjected to outlet obstruction -- an in vitro whole bladder study .
	manualset3
253389	2	425804	7	NULL	NULL	0	NULL	contractile function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation of contractile function and passive properties of rabbit urinary bladder subjected to outlet obstruction -- an in vitro whole bladder study .
	manualset3
253390	3	425804	7	NULL	NULL	0	NULL	passive properties	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation of contractile function and passive properties of rabbit urinary bladder subjected to outlet obstruction -- an in vitro whole bladder study .
	manualset3
253391	4	425804	7	NULL	NULL	0	NULL	rabbit urinary bladder	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation of contractile function and passive properties of rabbit urinary bladder subjected to outlet obstruction -- an in vitro whole bladder study .
	manualset3
253392	5	425804	7	NULL	NULL	0	NULL	 outlet obstruction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation of contractile function and passive properties of rabbit urinary bladder subjected to outlet obstruction -- an in vitro whole bladder study .
	manualset3
253393	6	425804	7	NULL	NULL	0	NULL	in vitro whole bladder study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation of contractile function and passive properties of rabbit urinary bladder subjected to outlet obstruction -- an in vitro whole bladder study .
	manualset3
253394	1	425805	7	NULL	NULL	0	NULL	Correlation 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation of pain relief with physical function in hand osteoarthritis : randomized controlled trial post hoc analysis .
	manualset3
253395	2	425805	7	NULL	NULL	0	NULL	 pain relief	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation of pain relief with physical function in hand osteoarthritis : randomized controlled trial post hoc analysis .
	manualset3
253396	3	425805	7	NULL	NULL	0	NULL	physical function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation of pain relief with physical function in hand osteoarthritis : randomized controlled trial post hoc analysis .
	manualset3
253397	4	425805	7	NULL	NULL	0	NULL	hand osteoarthritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation of pain relief with physical function in hand osteoarthritis : randomized controlled trial post hoc analysis .
	manualset3
253398	5	425805	7	NULL	NULL	0	NULL	randomized controlled trial	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation of pain relief with physical function in hand osteoarthritis : randomized controlled trial post hoc analysis .
	manualset3
253399	6	425805	7	NULL	NULL	0	NULL	post hoc analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlation of pain relief with physical function in hand osteoarthritis : randomized controlled trial post hoc analysis .
	manualset3
253400	1	425806	7	NULL	NULL	0	NULL	Correlations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlations between adiposity and maturity indicators are positive , but vary between r = 0.00 and r = 0.39 .
	manualset3
253401	2	425806	7	NULL	NULL	0	NULL	adiposity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlations between adiposity and maturity indicators are positive , but vary between r = 0.00 and r = 0.39 .
	manualset3
253402	3	425806	7	NULL	NULL	0	NULL	maturity indicators	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlations between adiposity and maturity indicators are positive , but vary between r = 0.00 and r = 0.39 .
	manualset3
253403	4	425806	7	NULL	NULL	0	NULL	r = 0.00	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlations between adiposity and maturity indicators are positive , but vary between r = 0.00 and r = 0.39 .
	manualset3
253404	5	425806	7	NULL	NULL	0	NULL	 r = 0.39	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlations between adiposity and maturity indicators are positive , but vary between r = 0.00 and r = 0.39 .
	manualset3
253405	1	425807	7	NULL	NULL	0	NULL	Correlations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlations between ultrasonography findings and hormonal profiles at oestrus in pure Spanish breed mares .
	manualset3
253406	2	425807	7	NULL	NULL	0	NULL	ultrasonography findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlations between ultrasonography findings and hormonal profiles at oestrus in pure Spanish breed mares .
	manualset3
253407	3	425807	7	NULL	NULL	0	NULL	hormonal profiles	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlations between ultrasonography findings and hormonal profiles at oestrus in pure Spanish breed mares .
	manualset3
253408	4	425807	7	NULL	NULL	0	NULL	oestrus	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlations between ultrasonography findings and hormonal profiles at oestrus in pure Spanish breed mares .
	manualset3
253409	5	425807	7	NULL	NULL	0	NULL	pure Spanish breed mares	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Correlations between ultrasonography findings and hormonal profiles at oestrus in pure Spanish breed mares .
	manualset3
253410	1	425808	7	NULL	NULL	0	NULL	Correspondence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Correspondence between judgments of learning ( JOLs ) and actual recall tends to be poor when the same items are studied and recalled multiple times ( e.g. , A. Koriat , L. Sheffer , & H. Ma'ayan , 2002 ) .
	manualset3
253411	2	425808	7	NULL	NULL	0	NULL	judgments of learning ( JOLs )	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Correspondence between judgments of learning ( JOLs ) and actual recall tends to be poor when the same items are studied and recalled multiple times ( e.g. , A. Koriat , L. Sheffer , & H. Ma'ayan , 2002 ) .
	manualset3
253412	3	425808	7	NULL	NULL	0	NULL	actual recall 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Correspondence between judgments of learning ( JOLs ) and actual recall tends to be poor when the same items are studied and recalled multiple times ( e.g. , A. Koriat , L. Sheffer , & H. Ma'ayan , 2002 ) .
	manualset3
253413	4	425808	7	NULL	NULL	0	NULL	same items	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Correspondence between judgments of learning ( JOLs ) and actual recall tends to be poor when the same items are studied and recalled multiple times ( e.g. , A. Koriat , L. Sheffer , & H. Ma'ayan , 2002 ) .
	manualset3
253414	5	425808	7	NULL	NULL	0	NULL	multiple times	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Correspondence between judgments of learning ( JOLs ) and actual recall tends to be poor when the same items are studied and recalled multiple times ( e.g. , A. Koriat , L. Sheffer , & H. Ma'ayan , 2002 ) .
	manualset3
253415	6	425808	7	NULL	NULL	0	NULL	A. Koriat , L. Sheffer , & H. Ma'ayan , 2002	PublicationOrCitation												NULL		0	NULL	NULL	NULL	NULL	NULL	Correspondence between judgments of learning ( JOLs ) and actual recall tends to be poor when the same items are studied and recalled multiple times ( e.g. , A. Koriat , L. Sheffer , & H. Ma'ayan , 2002 ) .
	manualset3
253416	1	425809	7	NULL	NULL	0	NULL	Corresponding photographic fields	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Corresponding photographic fields were graded by masked , trained graders for the severity of retinopathy and for the presence of specified diabetic lesions using the Modified Airlie House Classification scheme .
	manualset3
253417	2	425809	7	NULL	NULL	0	NULL	masked , trained graders	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Corresponding photographic fields were graded by masked , trained graders for the severity of retinopathy and for the presence of specified diabetic lesions using the Modified Airlie House Classification scheme .
	manualset3
253418	3	425809	7	NULL	NULL	0	NULL	severity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Corresponding photographic fields were graded by masked , trained graders for the severity of retinopathy and for the presence of specified diabetic lesions using the Modified Airlie House Classification scheme .
	manualset3
253419	4	425809	7	NULL	NULL	0	NULL	retinopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Corresponding photographic fields were graded by masked , trained graders for the severity of retinopathy and for the presence of specified diabetic lesions using the Modified Airlie House Classification scheme .
	manualset3
253420	5	425809	7	NULL	NULL	0	NULL	 presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Corresponding photographic fields were graded by masked , trained graders for the severity of retinopathy and for the presence of specified diabetic lesions using the Modified Airlie House Classification scheme .
	manualset3
253421	6	425809	7	NULL	NULL	0	NULL	 diabetic lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Corresponding photographic fields were graded by masked , trained graders for the severity of retinopathy and for the presence of specified diabetic lesions using the Modified Airlie House Classification scheme .
	manualset3
253422	7	425809	7	NULL	NULL	0	NULL	Modified Airlie House Classification scheme	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Corresponding photographic fields were graded by masked , trained graders for the severity of retinopathy and for the presence of specified diabetic lesions using the Modified Airlie House Classification scheme .
	manualset3
253423	1	425810	7	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Corresponding to the increase in CF concentrations from 0.1 to 0.3 wt % , the average IB and Nakagami parameter ( m ) of the composite samples increased from -78.10 2.20 ( mean standard deviation ) to -72.66 1.40 dB and from 0.024 0.012 to 0.048 0.011 , respectively .
	manualset3
253424	2	425810	7	NULL	NULL	0	NULL	CF concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Corresponding to the increase in CF concentrations from 0.1 to 0.3 wt % , the average IB and Nakagami parameter ( m ) of the composite samples increased from -78.10 2.20 ( mean standard deviation ) to -72.66 1.40 dB and from 0.024 0.012 to 0.048 0.011 , respectively .
	manualset3
253425	3	425810	7	NULL	NULL	0	NULL	 0.1%	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Corresponding to the increase in CF concentrations from 0.1 to 0.3 wt % , the average IB and Nakagami parameter ( m ) of the composite samples increased from -78.10 2.20 ( mean standard deviation ) to -72.66 1.40 dB and from 0.024 0.012 to 0.048 0.011 , respectively .
	manualset3
253426	4	425810	7	NULL	NULL	0	NULL	0.3 wt %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Corresponding to the increase in CF concentrations from 0.1 to 0.3 wt % , the average IB and Nakagami parameter ( m ) of the composite samples increased from -78.10 2.20 ( mean standard deviation ) to -72.66 1.40 dB and from 0.024 0.012 to 0.048 0.011 , respectively .
	manualset3
253427	5	425810	7	NULL	NULL	0	NULL	average IB	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Corresponding to the increase in CF concentrations from 0.1 to 0.3 wt % , the average IB and Nakagami parameter ( m ) of the composite samples increased from -78.10 2.20 ( mean standard deviation ) to -72.66 1.40 dB and from 0.024 0.012 to 0.048 0.011 , respectively .
	manualset3
253428	6	425810	7	NULL	NULL	0	NULL	Nakagami parameter ( m )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Corresponding to the increase in CF concentrations from 0.1 to 0.3 wt % , the average IB and Nakagami parameter ( m ) of the composite samples increased from -78.10 2.20 ( mean standard deviation ) to -72.66 1.40 dB and from 0.024 0.012 to 0.048 0.011 , respectively .
	manualset3
253429	7	425810	7	NULL	NULL	0	NULL	composite samples	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Corresponding to the increase in CF concentrations from 0.1 to 0.3 wt % , the average IB and Nakagami parameter ( m ) of the composite samples increased from -78.10 2.20 ( mean standard deviation ) to -72.66 1.40 dB and from 0.024 0.012 to 0.048 0.011 , respectively .
	manualset3
253430	8	425810	7	NULL	NULL	0	NULL	-78.10 2.20	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Corresponding to the increase in CF concentrations from 0.1 to 0.3 wt % , the average IB and Nakagami parameter ( m ) of the composite samples increased from -78.10 2.20 ( mean standard deviation ) to -72.66 1.40 dB and from 0.024 0.012 to 0.048 0.011 , respectively .
	manualset3
253431	9	425810	7	NULL	NULL	0	NULL	mean standard deviation 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Corresponding to the increase in CF concentrations from 0.1 to 0.3 wt % , the average IB and Nakagami parameter ( m ) of the composite samples increased from -78.10 2.20 ( mean standard deviation ) to -72.66 1.40 dB and from 0.024 0.012 to 0.048 0.011 , respectively .
	manualset3
253432	10	425810	7	NULL	NULL	0	NULL	-72.66 1.40 dB	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Corresponding to the increase in CF concentrations from 0.1 to 0.3 wt % , the average IB and Nakagami parameter ( m ) of the composite samples increased from -78.10 2.20 ( mean standard deviation ) to -72.66 1.40 dB and from 0.024 0.012 to 0.048 0.011 , respectively .
	manualset3
253433	11	425810	7	NULL	NULL	0	NULL	 0.024 0.012 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Corresponding to the increase in CF concentrations from 0.1 to 0.3 wt % , the average IB and Nakagami parameter ( m ) of the composite samples increased from -78.10 2.20 ( mean standard deviation ) to -72.66 1.40 dB and from 0.024 0.012 to 0.048 0.011 , respectively .
	manualset3
253434	12	425810	7	NULL	NULL	0	NULL	 0.048 0.011	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Corresponding to the increase in CF concentrations from 0.1 to 0.3 wt % , the average IB and Nakagami parameter ( m ) of the composite samples increased from -78.10 2.20 ( mean standard deviation ) to -72.66 1.40 dB and from 0.024 0.012 to 0.048 0.011 , respectively .
	manualset3
253435	1	425811	7	NULL	NULL	0	NULL	synergistic effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Correspondingly , a synergistic effect of T 3 with the same concentration and GH on cell proliferation in human adult osteoblast-like cells was found .
	manualset3
253436	2	425811	7	NULL	NULL	0	NULL	T3	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Correspondingly , a synergistic effect of T 3 with the same concentration and GH on cell proliferation in human adult osteoblast-like cells was found .
	manualset3
253437	3	425811	7	NULL	NULL	0	NULL	concentration	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Correspondingly , a synergistic effect of T 3 with the same concentration and GH on cell proliferation in human adult osteoblast-like cells was found .
	manualset3
253438	4	425811	7	NULL	NULL	0	NULL	GH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Correspondingly , a synergistic effect of T 3 with the same concentration and GH on cell proliferation in human adult osteoblast-like cells was found .
	manualset3
253439	5	425811	7	NULL	NULL	0	NULL	cell proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Correspondingly , a synergistic effect of T 3 with the same concentration and GH on cell proliferation in human adult osteoblast-like cells was found .
	manualset3
253440	6	425811	7	NULL	NULL	0	NULL	human adult osteoblast-like cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Correspondingly , a synergistic effect of T 3 with the same concentration and GH on cell proliferation in human adult osteoblast-like cells was found .
	manualset3
253441	1	425812	7	NULL	NULL	0	NULL	Corticosteroid recoveries	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Corticosteroid recoveries were 73 % , 74 % , and 90 % for prednisolone , prednisone , and cortisol , respectively .
	manualset3
253442	2	425812	7	NULL	NULL	0	NULL	73 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Corticosteroid recoveries were 73 % , 74 % , and 90 % for prednisolone , prednisone , and cortisol , respectively .
	manualset3
253443	3	425812	7	NULL	NULL	0	NULL	74 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Corticosteroid recoveries were 73 % , 74 % , and 90 % for prednisolone , prednisone , and cortisol , respectively .
	manualset3
253444	4	425812	7	NULL	NULL	0	NULL	90 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Corticosteroid recoveries were 73 % , 74 % , and 90 % for prednisolone , prednisone , and cortisol , respectively .
	manualset3
253445	5	425812	7	NULL	NULL	NULL	NULL	prednisolone	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Corticosteroid recoveries were 73 % , 74 % , and 90 % for prednisolone , prednisone , and cortisol , respectively .
	manualset3
253446	6	425812	7	NULL	NULL	NULL	NULL	prednisone	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Corticosteroid recoveries were 73 % , 74 % , and 90 % for prednisolone , prednisone , and cortisol , respectively .
	manualset3
253447	7	425812	7	NULL	NULL	0	NULL	cortisol 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Corticosteroid recoveries were 73 % , 74 % , and 90 % for prednisolone , prednisone , and cortisol , respectively .
	manualset3
253449	1	425813	7	NULL	NULL	0	NULL	Malignant bile duct diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Malignant bile duct diseases and jaundice ) .
	manualset3
253450	2	425813	7	NULL	NULL	0	NULL	jaundice 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Malignant bile duct diseases and jaundice ) .
	manualset3
253451	1	425814	7	NULL	NULL	0	NULL	Cortisol	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Cortisol is used in research as a biomarker of psychological stress .
	manualset3
253452	2	425814	7	NULL	NULL	0	NULL	 research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Cortisol is used in research as a biomarker of psychological stress .
	manualset3
253453	3	425814	7	NULL	NULL	0	NULL	biomarker	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Cortisol is used in research as a biomarker of psychological stress .
	manualset3
253454	4	425814	7	NULL	NULL	0	NULL	 psychological stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Cortisol is used in research as a biomarker of psychological stress .
	manualset3
253455	1	425815	7	NULL	NULL	0	NULL	Cortisol response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Cortisol response and immune-related effects of Atlantic salmon ( Salmo salar Linnaeus ) subjected to short - and long-term stress .
	manualset3
253456	2	425815	7	NULL	NULL	0	NULL	immune-related effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Cortisol response and immune-related effects of Atlantic salmon ( Salmo salar Linnaeus ) subjected to short - and long-term stress .
	manualset3
253457	3	425815	7	NULL	NULL	0	NULL	Atlantic salmon	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Cortisol response and immune-related effects of Atlantic salmon ( Salmo salar Linnaeus ) subjected to short - and long-term stress .
	manualset3
253458	4	425815	7	NULL	NULL	0	NULL	Salmo salar Linnaeus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Cortisol response and immune-related effects of Atlantic salmon ( Salmo salar Linnaeus ) subjected to short - and long-term stress .
	manualset3
253459	5	425815	7	NULL	NULL	0	NULL	 short -stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Cortisol response and immune-related effects of Atlantic salmon ( Salmo salar Linnaeus ) subjected to short - and long-term stress .
	manualset3
253460	6	425815	7	NULL	NULL	0	NULL	long-term stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Cortisol response and immune-related effects of Atlantic salmon ( Salmo salar Linnaeus ) subjected to short - and long-term stress .
	manualset3
253723	1	425816	7	NULL	NULL	NULL	NULL	Cost-benefit analysis	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cost-benefit analysis of selective screening criteria for Chlamydia trachomatis infection in women attending Colorado family planning clinics .
	manualset3
253724	2	425816	7	NULL	NULL	NULL	NULL	selective screening criteria	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cost-benefit analysis of selective screening criteria for Chlamydia trachomatis infection in women attending Colorado family planning clinics .
	manualset3
253725	3	425816	7	NULL	NULL	NULL	NULL	Chlamydia trachomatis infection	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cost-benefit analysis of selective screening criteria for Chlamydia trachomatis infection in women attending Colorado family planning clinics .
	manualset3
253726	4	425816	7	NULL	NULL	NULL	NULL	women	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cost-benefit analysis of selective screening criteria for Chlamydia trachomatis infection in women attending Colorado family planning clinics .
	manualset3
253727	5	425816	7	NULL	NULL	NULL	NULL	Colorado family planning clinics	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cost-benefit analysis of selective screening criteria for Chlamydia trachomatis infection in women attending Colorado family planning clinics .
	manualset3
253728	1	425817	7	NULL	NULL	NULL	NULL	Cost-of-illness studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cost-of-illness studies in systemic lupus erythematosus : A systematic review .
	manualset3
253729	2	425817	7	NULL	NULL	NULL	NULL	systemic lupus erythematosus	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cost-of-illness studies in systemic lupus erythematosus : A systematic review .
	manualset3
253730	3	425817	7	NULL	NULL	NULL	NULL	systematic review	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cost-of-illness studies in systemic lupus erythematosus : A systematic review .
	manualset3
253731	1	425818	7	NULL	NULL	NULL	NULL	Cost analysis 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cost analysis of kidney-pancreas and kidney-islet transplant .
	manualset3
253732	2	425818	7	NULL	NULL	NULL	NULL	 kidney-pancreas	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cost analysis of kidney-pancreas and kidney-islet transplant .
	manualset3
253733	3	425818	7	NULL	NULL	NULL	NULL	kidney-islet transplant	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cost analysis of kidney-pancreas and kidney-islet transplant .
	manualset3
253734	1	425819	7	NULL	NULL	NULL	NULL	Malignant mesothelioma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Malignant mesothelioma of the pleura ( author 's transl ) ) .
	manualset3
253735	2	425819	7	NULL	NULL	NULL	NULL	pleura	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Malignant mesothelioma of the pleura ( author 's transl ) ) .
	manualset3
253736	3	425819	7	NULL	NULL	NULL	NULL	author 's transl	PublicationOrCitation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Malignant mesothelioma of the pleura ( author 's transl ) ) .
	manualset3
253737	1	425820	7	NULL	NULL	NULL	NULL	Costing studies 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Costing studies showed that up to 75 % of the total expenditure of the agency in 2010 was spent on public health services subject to external audit or certification .
	manualset3
253738	2	425820	7	NULL	NULL	NULL	NULL	75 %	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Costing studies showed that up to 75 % of the total expenditure of the agency in 2010 was spent on public health services subject to external audit or certification .
	manualset3
253739	3	425820	7	NULL	NULL	NULL	NULL	total expenditure	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Costing studies showed that up to 75 % of the total expenditure of the agency in 2010 was spent on public health services subject to external audit or certification .
	manualset3
253740	4	425820	7	NULL	NULL	NULL	NULL	 agency	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Costing studies showed that up to 75 % of the total expenditure of the agency in 2010 was spent on public health services subject to external audit or certification .
	manualset3
253741	5	425820	7	NULL	NULL	NULL	NULL	 2010 	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Costing studies showed that up to 75 % of the total expenditure of the agency in 2010 was spent on public health services subject to external audit or certification .
	manualset3
253742	6	425820	7	NULL	NULL	NULL	NULL	public health services	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Costing studies showed that up to 75 % of the total expenditure of the agency in 2010 was spent on public health services subject to external audit or certification .
	manualset3
253743	7	425820	7	NULL	NULL	NULL	NULL	 external audit	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Costing studies showed that up to 75 % of the total expenditure of the agency in 2010 was spent on public health services subject to external audit or certification .
	manualset3
253744	8	425820	7	NULL	NULL	NULL	NULL	certification	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Costing studies showed that up to 75 % of the total expenditure of the agency in 2010 was spent on public health services subject to external audit or certification .
	manualset3
253775	1	425821	7	NULL	NULL	NULL	NULL	Cotransfection analyses 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cotransfection analyses demonstrated that NKX-3 .1 can abolish the transcriptional activation function of PDEF on the prostate-specific antigen ( PSA ) promoter .
	manualset3
253778	2	425821	7	NULL	NULL	NULL	NULL	NKX-3 .1	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cotransfection analyses demonstrated that NKX-3 .1 can abolish the transcriptional activation function of PDEF on the prostate-specific antigen ( PSA ) promoter .
	manualset3
253779	3	425821	7	NULL	NULL	NULL	NULL	transcriptional activation function	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cotransfection analyses demonstrated that NKX-3 .1 can abolish the transcriptional activation function of PDEF on the prostate-specific antigen ( PSA ) promoter .
	manualset3
253797	4	425821	7	NULL	NULL	NULL	NULL	PDEF	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cotransfection analyses demonstrated that NKX-3 .1 can abolish the transcriptional activation function of PDEF on the prostate-specific antigen ( PSA ) promoter .
	manualset3
253799	5	425821	7	NULL	NULL	NULL	NULL	prostate-specific antigen ( PSA ) promoter	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cotransfection analyses demonstrated that NKX-3 .1 can abolish the transcriptional activation function of PDEF on the prostate-specific antigen ( PSA ) promoter .
	manualset3
253816	1	425822	7	NULL	NULL	NULL	NULL	Cotransplantation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cotransplantation of MSCs and hematopoietic stem cells ( HSCs ) from HLA-identical siblings has been shown to reduce the incidence of acute graft-vs .
	manualset3
253817	2	425822	7	NULL	NULL	NULL	NULL	MSCs	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cotransplantation of MSCs and hematopoietic stem cells ( HSCs ) from HLA-identical siblings has been shown to reduce the incidence of acute graft-vs .
	manualset3
253819	3	425822	7	NULL	NULL	NULL	NULL	hematopoietic stem cells ( HSCs )	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cotransplantation of MSCs and hematopoietic stem cells ( HSCs ) from HLA-identical siblings has been shown to reduce the incidence of acute graft-vs .
	manualset3
253821	4	425822	7	NULL	NULL	NULL	NULL	HLA-identical siblings	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cotransplantation of MSCs and hematopoietic stem cells ( HSCs ) from HLA-identical siblings has been shown to reduce the incidence of acute graft-vs .
	manualset3
253825	5	425822	7	NULL	NULL	NULL	NULL	 incidence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cotransplantation of MSCs and hematopoietic stem cells ( HSCs ) from HLA-identical siblings has been shown to reduce the incidence of acute graft-vs .
	manualset3
253831	6	425822	7	NULL	NULL	NULL	NULL	acute graft	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cotransplantation of MSCs and hematopoietic stem cells ( HSCs ) from HLA-identical siblings has been shown to reduce the incidence of acute graft-vs .
	manualset3
253896	1	425823	7	NULL	NULL	NULL	NULL	Cotreatment 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cotreatment of GLCs with CS and aminoglutethimide , an aromatase inhibitor , completely abolished CS-induced E2 production .
	manualset3
253905	2	425823	7	NULL	NULL	NULL	NULL	GLCs	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cotreatment of GLCs with CS and aminoglutethimide , an aromatase inhibitor , completely abolished CS-induced E2 production .
	manualset3
253906	3	425823	7	NULL	NULL	NULL	NULL	 CS	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cotreatment of GLCs with CS and aminoglutethimide , an aromatase inhibitor , completely abolished CS-induced E2 production .
	manualset3
253907	4	425823	7	NULL	NULL	NULL	NULL	aminoglutethimide	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cotreatment of GLCs with CS and aminoglutethimide , an aromatase inhibitor , completely abolished CS-induced E2 production .
	manualset3
253908	5	425823	7	NULL	NULL	NULL	NULL	 aromatase inhibitor	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cotreatment of GLCs with CS and aminoglutethimide , an aromatase inhibitor , completely abolished CS-induced E2 production .
	manualset3
253909	6	425823	7	NULL	NULL	NULL	NULL	CS-induced E2 production	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cotreatment of GLCs with CS and aminoglutethimide , an aromatase inhibitor , completely abolished CS-induced E2 production .
	manualset3
253913	1	425824	7	NULL	NULL	NULL	NULL	Cotyledonary arteriole diameters	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cotyledonary arteriole diameters were markedly greater ( P & lt ; 0.05 ) in OB than C ewes at MG , but while arteriole diameter of C ewes increased ( P & lt ; 0.05 ) from MG to LG , they remained unchanged in OB ewes .
	manualset3
253914	2	425824	7	NULL	NULL	NULL	NULL	P & lt ; 0.05	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cotyledonary arteriole diameters were markedly greater ( P & lt ; 0.05 ) in OB than C ewes at MG , but while arteriole diameter of C ewes increased ( P & lt ; 0.05 ) from MG to LG , they remained unchanged in OB ewes .
	manualset3
253930	3	425824	7	NULL	NULL	NULL	NULL	OB ewes	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cotyledonary arteriole diameters were markedly greater ( P & lt ; 0.05 ) in OB than C ewes at MG , but while arteriole diameter of C ewes increased ( P & lt ; 0.05 ) from MG to LG , they remained unchanged in OB ewes .
	manualset3
253935	4	425824	7	NULL	NULL	NULL	NULL	C ewes	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cotyledonary arteriole diameters were markedly greater ( P & lt ; 0.05 ) in OB than C ewes at MG , but while arteriole diameter of C ewes increased ( P & lt ; 0.05 ) from MG to LG , they remained unchanged in OB ewes .
	manualset3
253938	5	425824	7	NULL	NULL	NULL	NULL	MG	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cotyledonary arteriole diameters were markedly greater ( P & lt ; 0.05 ) in OB than C ewes at MG , but while arteriole diameter of C ewes increased ( P & lt ; 0.05 ) from MG to LG , they remained unchanged in OB ewes .
	manualset3
253939	6	425824	7	NULL	NULL	NULL	NULL	arteriole diameter	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cotyledonary arteriole diameters were markedly greater ( P & lt ; 0.05 ) in OB than C ewes at MG , but while arteriole diameter of C ewes increased ( P & lt ; 0.05 ) from MG to LG , they remained unchanged in OB ewes .
	manualset3
253942	7	425824	7	NULL	NULL	NULL	NULL	C ewes	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cotyledonary arteriole diameters were markedly greater ( P & lt ; 0.05 ) in OB than C ewes at MG , but while arteriole diameter of C ewes increased ( P & lt ; 0.05 ) from MG to LG , they remained unchanged in OB ewes .
	manualset3
253943	8	425824	7	NULL	NULL	NULL	NULL	P & lt ; 0.05	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cotyledonary arteriole diameters were markedly greater ( P & lt ; 0.05 ) in OB than C ewes at MG , but while arteriole diameter of C ewes increased ( P & lt ; 0.05 ) from MG to LG , they remained unchanged in OB ewes .
	manualset3
253945	9	425824	7	NULL	NULL	NULL	NULL	MG	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cotyledonary arteriole diameters were markedly greater ( P & lt ; 0.05 ) in OB than C ewes at MG , but while arteriole diameter of C ewes increased ( P & lt ; 0.05 ) from MG to LG , they remained unchanged in OB ewes .
	manualset3
253947	10	425824	7	NULL	NULL	NULL	NULL	LG	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cotyledonary arteriole diameters were markedly greater ( P & lt ; 0.05 ) in OB than C ewes at MG , but while arteriole diameter of C ewes increased ( P & lt ; 0.05 ) from MG to LG , they remained unchanged in OB ewes .
	manualset3
253951	11	425824	7	NULL	NULL	NULL	NULL	OB ewes	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cotyledonary arteriole diameters were markedly greater ( P & lt ; 0.05 ) in OB than C ewes at MG , but while arteriole diameter of C ewes increased ( P & lt ; 0.05 ) from MG to LG , they remained unchanged in OB ewes .
	manualset3
254008	1	425825	7	NULL	NULL	NULL	NULL	Massive hemoptysis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Massive hemoptysis caused by disruption of a bronchial aneurysm diagnosed by microscopic examination of the resected lung ) .
	manualset3
254010	2	425825	7	NULL	NULL	NULL	NULL	disruption	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Massive hemoptysis caused by disruption of a bronchial aneurysm diagnosed by microscopic examination of the resected lung ) .
	manualset3
254011	3	425825	7	NULL	NULL	NULL	NULL	bronchial aneurysm	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Massive hemoptysis caused by disruption of a bronchial aneurysm diagnosed by microscopic examination of the resected lung ) .
	manualset3
254013	4	425825	7	NULL	NULL	NULL	NULL	microscopic examination	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Massive hemoptysis caused by disruption of a bronchial aneurysm diagnosed by microscopic examination of the resected lung ) .
	manualset3
254015	5	425825	7	NULL	NULL	NULL	NULL	resected lung	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Massive hemoptysis caused by disruption of a bronchial aneurysm diagnosed by microscopic examination of the resected lung ) .
	manualset3
254019	1	425826	7	NULL	NULL	NULL	NULL	Count rate losses	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Count rate losses due to pulse pile-up , image contamination due to acceptance of random coincidences and Compton scatter , and image artifacts produced by photon attenuation were measured .
	manualset3
254021	2	425826	7	NULL	NULL	NULL	NULL	pulse pile-up 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Count rate losses due to pulse pile-up , image contamination due to acceptance of random coincidences and Compton scatter , and image artifacts produced by photon attenuation were measured .
	manualset3
254022	3	425826	7	NULL	NULL	NULL	NULL	image contamination	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Count rate losses due to pulse pile-up , image contamination due to acceptance of random coincidences and Compton scatter , and image artifacts produced by photon attenuation were measured .
	manualset3
254023	4	425826	7	NULL	NULL	NULL	NULL	acceptance	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Count rate losses due to pulse pile-up , image contamination due to acceptance of random coincidences and Compton scatter , and image artifacts produced by photon attenuation were measured .
	manualset3
254025	5	425826	7	NULL	NULL	NULL	NULL	random coincidences	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Count rate losses due to pulse pile-up , image contamination due to acceptance of random coincidences and Compton scatter , and image artifacts produced by photon attenuation were measured .
	manualset3
254026	6	425826	7	NULL	NULL	NULL	NULL	Compton scatter	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Count rate losses due to pulse pile-up , image contamination due to acceptance of random coincidences and Compton scatter , and image artifacts produced by photon attenuation were measured .
	manualset3
254027	7	425826	7	NULL	NULL	NULL	NULL	image artifacts	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Count rate losses due to pulse pile-up , image contamination due to acceptance of random coincidences and Compton scatter , and image artifacts produced by photon attenuation were measured .
	manualset3
254028	8	425826	7	NULL	NULL	NULL	NULL	photon attenuation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Count rate losses due to pulse pile-up , image contamination due to acceptance of random coincidences and Compton scatter , and image artifacts produced by photon attenuation were measured .
	manualset3
254030	1	425827	7	NULL	NULL	NULL	NULL	hypothesis	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Counter to our hypothesis , isoproterenol-mediated airway relaxation was significantly attenuated ( 50 % ) in AC5-TG , as was cAMP production , suggesting compensatory regulatory events limiting ( 2 ) - AR signaling when AC expression is increased .
	manualset3
254031	2	425827	7	NULL	NULL	NULL	NULL	isoproterenol-mediated airway relaxation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Counter to our hypothesis , isoproterenol-mediated airway relaxation was significantly attenuated ( 50 % ) in AC5-TG , as was cAMP production , suggesting compensatory regulatory events limiting ( 2 ) - AR signaling when AC expression is increased .
	manualset3
254032	3	425827	7	NULL	NULL	NULL	NULL	50 % 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Counter to our hypothesis , isoproterenol-mediated airway relaxation was significantly attenuated ( 50 % ) in AC5-TG , as was cAMP production , suggesting compensatory regulatory events limiting ( 2 ) - AR signaling when AC expression is increased .
	manualset3
254033	4	425827	7	NULL	NULL	NULL	NULL	AC5-TG	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Counter to our hypothesis , isoproterenol-mediated airway relaxation was significantly attenuated ( 50 % ) in AC5-TG , as was cAMP production , suggesting compensatory regulatory events limiting ( 2 ) - AR signaling when AC expression is increased .
	manualset3
254034	5	425827	7	NULL	NULL	NULL	NULL	cAMP production	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Counter to our hypothesis , isoproterenol-mediated airway relaxation was significantly attenuated ( 50 % ) in AC5-TG , as was cAMP production , suggesting compensatory regulatory events limiting ( 2 ) - AR signaling when AC expression is increased .
	manualset3
254035	6	425827	7	NULL	NULL	NULL	NULL	regulatory events 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Counter to our hypothesis , isoproterenol-mediated airway relaxation was significantly attenuated ( 50 % ) in AC5-TG , as was cAMP production , suggesting compensatory regulatory events limiting ( 2 ) - AR signaling when AC expression is increased .
	manualset3
254037	7	425827	7	NULL	NULL	NULL	NULL	( 2 ) - AR signaling 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Counter to our hypothesis , isoproterenol-mediated airway relaxation was significantly attenuated ( 50 % ) in AC5-TG , as was cAMP production , suggesting compensatory regulatory events limiting ( 2 ) - AR signaling when AC expression is increased .
	manualset3
254038	8	425827	7	NULL	NULL	NULL	NULL	AC expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Counter to our hypothesis , isoproterenol-mediated airway relaxation was significantly attenuated ( 50 % ) in AC5-TG , as was cAMP production , suggesting compensatory regulatory events limiting ( 2 ) - AR signaling when AC expression is increased .
	manualset3
254043	1	425828	7	NULL	NULL	NULL	NULL	Counteracting postsurgical adhesions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Counteracting postsurgical adhesions -- the effect of combining oxidized regenerated cellulose and tissue plasminogen activator .
	manualset3
254045	2	425828	7	NULL	NULL	NULL	NULL	effect	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Counteracting postsurgical adhesions -- the effect of combining oxidized regenerated cellulose and tissue plasminogen activator .
	manualset3
254047	3	425828	7	NULL	NULL	NULL	NULL	oxidized regenerated cellulose	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Counteracting postsurgical adhesions -- the effect of combining oxidized regenerated cellulose and tissue plasminogen activator .
	manualset3
254048	4	425828	7	NULL	NULL	NULL	NULL	tissue plasminogen activator	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Counteracting postsurgical adhesions -- the effect of combining oxidized regenerated cellulose and tissue plasminogen activator .
	manualset3
254058	1	425829	7	NULL	NULL	NULL	NULL	Counts	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Counts were made of eggs laid on Styrofoam blocks , container sides , and water surface , and dissections allowed for counts of retained eggs to determine the fecundity of this species .
	manualset3
254059	2	425829	7	NULL	NULL	NULL	NULL	eggs	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Counts were made of eggs laid on Styrofoam blocks , container sides , and water surface , and dissections allowed for counts of retained eggs to determine the fecundity of this species .
	manualset3
254061	3	425829	7	NULL	NULL	NULL	NULL	 Styrofoam blocks	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Counts were made of eggs laid on Styrofoam blocks , container sides , and water surface , and dissections allowed for counts of retained eggs to determine the fecundity of this species .
	manualset3
254062	4	425829	7	NULL	NULL	NULL	NULL	container sides	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Counts were made of eggs laid on Styrofoam blocks , container sides , and water surface , and dissections allowed for counts of retained eggs to determine the fecundity of this species .
	manualset3
254063	5	425829	7	NULL	NULL	NULL	NULL	water surface	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Counts were made of eggs laid on Styrofoam blocks , container sides , and water surface , and dissections allowed for counts of retained eggs to determine the fecundity of this species .
	manualset3
254064	6	425829	7	NULL	NULL	NULL	NULL	dissections	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Counts were made of eggs laid on Styrofoam blocks , container sides , and water surface , and dissections allowed for counts of retained eggs to determine the fecundity of this species .
	manualset3
254065	7	425829	7	NULL	NULL	NULL	NULL	counts	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Counts were made of eggs laid on Styrofoam blocks , container sides , and water surface , and dissections allowed for counts of retained eggs to determine the fecundity of this species .
	manualset3
254067	8	425829	7	NULL	NULL	NULL	NULL	retained eggs	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Counts were made of eggs laid on Styrofoam blocks , container sides , and water surface , and dissections allowed for counts of retained eggs to determine the fecundity of this species .
	manualset3
254068	9	425829	7	NULL	NULL	NULL	NULL	fecundity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Counts were made of eggs laid on Styrofoam blocks , container sides , and water surface , and dissections allowed for counts of retained eggs to determine the fecundity of this species .
	manualset3
254070	10	425829	7	NULL	NULL	NULL	NULL	species	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Counts were made of eggs laid on Styrofoam blocks , container sides , and water surface , and dissections allowed for counts of retained eggs to determine the fecundity of this species .
	manualset3
254073	1	425830	7	NULL	NULL	NULL	NULL	variability	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coupled to this variability in estrogen is an equally variable set of changes in progesterone secretion by the ovary as androgen secretion patterns also change .
	manualset3
254074	2	425830	7	NULL	NULL	NULL	NULL	estrogen	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coupled to this variability in estrogen is an equally variable set of changes in progesterone secretion by the ovary as androgen secretion patterns also change .
	manualset3
254075	3	425830	7	NULL	NULL	NULL	NULL	variable set 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coupled to this variability in estrogen is an equally variable set of changes in progesterone secretion by the ovary as androgen secretion patterns also change .
	manualset3
254076	4	425830	7	NULL	NULL	NULL	NULL	changes	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coupled to this variability in estrogen is an equally variable set of changes in progesterone secretion by the ovary as androgen secretion patterns also change .
	manualset3
254077	5	425830	7	NULL	NULL	NULL	NULL	progesterone secretion	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coupled to this variability in estrogen is an equally variable set of changes in progesterone secretion by the ovary as androgen secretion patterns also change .
	manualset3
254078	6	425830	7	NULL	NULL	NULL	NULL	 ovary	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coupled to this variability in estrogen is an equally variable set of changes in progesterone secretion by the ovary as androgen secretion patterns also change .
	manualset3
254079	7	425830	7	NULL	NULL	NULL	NULL	androgen secretion patterns	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coupled to this variability in estrogen is an equally variable set of changes in progesterone secretion by the ovary as androgen secretion patterns also change .
	manualset3
254421	1	425831	7	NULL	NULL	NULL	NULL	Couples 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Couples coping in response to kidney disease : a developmental perspective .
	manualset3
254423	2	425831	7	NULL	NULL	NULL	NULL	kidney disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Couples coping in response to kidney disease : a developmental perspective .
	manualset3
254426	3	425831	7	NULL	NULL	NULL	NULL	developmental perspective	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Couples coping in response to kidney disease : a developmental perspective .
	manualset3
258824	4	425831	7	NULL	NULL	NULL	NULL	response	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Couples coping in response to kidney disease : a developmental perspective .
	manualset3
254627	1	425832	7	NULL	NULL	NULL	NULL	Coupling polymerase pausing	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coupling polymerase pausing and chromatin landscapes for precise regulation of transcription .
	manualset3
254628	2	425832	7	NULL	NULL	NULL	NULL	chromatin landscapes	Chromosome												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coupling polymerase pausing and chromatin landscapes for precise regulation of transcription .
	manualset3
254629	3	425832	7	NULL	NULL	NULL	NULL	regulation 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coupling polymerase pausing and chromatin landscapes for precise regulation of transcription .
	manualset3
254630	4	425832	7	NULL	NULL	NULL	NULL	transcription 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coupling polymerase pausing and chromatin landscapes for precise regulation of transcription .
	manualset3
254631	1	425833	7	NULL	NULL	NULL	NULL	Courts	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Courts , in keeping with a tradition of self-determination , continue to protect a patient 's right to decide whether his or her life has quality enough to prolong it .
	manualset3
254632	2	425833	7	NULL	NULL	NULL	NULL	tradition	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Courts , in keeping with a tradition of self-determination , continue to protect a patient 's right to decide whether his or her life has quality enough to prolong it .
	manualset3
254633	3	425833	7	NULL	NULL	NULL	NULL	self-determination	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Courts , in keeping with a tradition of self-determination , continue to protect a patient 's right to decide whether his or her life has quality enough to prolong it .
	manualset3
254634	4	425833	7	NULL	NULL	NULL	NULL	 patient 's right	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Courts , in keeping with a tradition of self-determination , continue to protect a patient 's right to decide whether his or her life has quality enough to prolong it .
	manualset3
254636	5	425833	7	NULL	NULL	NULL	NULL	quality	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Courts , in keeping with a tradition of self-determination , continue to protect a patient 's right to decide whether his or her life has quality enough to prolong it .
	manualset3
258597	6	425833	7	NULL	NULL	NULL	NULL	life	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Courts , in keeping with a tradition of self-determination , continue to protect a patient 's right to decide whether his or her life has quality enough to prolong it .
	manualset3
254637	1	425834	7	NULL	NULL	NULL	NULL	Covalently bound radioactivity	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Covalently bound radioactivity was found exclusively on the light chain .
	manualset3
254638	2	425834	7	NULL	NULL	NULL	NULL	 light chain 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Covalently bound radioactivity was found exclusively on the light chain .
	manualset3
254640	1	425835	7	NULL	NULL	NULL	NULL	1000th Anniversary	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( 1000th Anniversary of Avicenna 's birth ) .
	manualset3
254643	2	425835	7	NULL	NULL	NULL	NULL	Avicenna 's birth	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( 1000th Anniversary of Avicenna 's birth ) .
	manualset3
254645	1	425836	7	NULL	NULL	NULL	NULL	Massive multifocal echinococcosis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Massive multifocal echinococcosis ) .
	manualset3
254647	1	425837	7	NULL	NULL	NULL	NULL	Coverage	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coverage by attending radiologists around the clock is expensive and difficult to implement .
	manualset3
254649	2	425837	7	NULL	NULL	NULL	NULL	radiologists	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coverage by attending radiologists around the clock is expensive and difficult to implement .
	manualset3
254650	3	425837	7	NULL	NULL	NULL	NULL	clock	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coverage by attending radiologists around the clock is expensive and difficult to implement .
	manualset3
254651	1	425838	7	NULL	NULL	NULL	NULL	Cowpea mosaic virus ( CPMV )	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cowpea mosaic virus ( CPMV ) is a bipartite RNA plant virus which has proved to be useful both for epitope presentation and as a polypeptide expression system .
	manualset3
254652	2	425838	7	NULL	NULL	NULL	NULL	bipartite RNA plant virus	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cowpea mosaic virus ( CPMV ) is a bipartite RNA plant virus which has proved to be useful both for epitope presentation and as a polypeptide expression system .
	manualset3
254654	3	425838	7	NULL	NULL	NULL	NULL	epitope presentation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cowpea mosaic virus ( CPMV ) is a bipartite RNA plant virus which has proved to be useful both for epitope presentation and as a polypeptide expression system .
	manualset3
254655	4	425838	7	NULL	NULL	NULL	NULL	polypeptide expression system	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cowpea mosaic virus ( CPMV ) is a bipartite RNA plant virus which has proved to be useful both for epitope presentation and as a polypeptide expression system .
	manualset3
254656	1	425839	7	NULL	NULL	NULL	NULL	Coxsackievirus A2 ( CAV2 )	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coxsackievirus A2 ( CAV2 ) , CBV2 , CBV5 , E7 , E11 , E19 , E24 , E29 and enterovirus 71 were recovered only from sporadic cases .
	manualset3
254657	2	425839	7	NULL	NULL	NULL	NULL	CBV2	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coxsackievirus A2 ( CAV2 ) , CBV2 , CBV5 , E7 , E11 , E19 , E24 , E29 and enterovirus 71 were recovered only from sporadic cases .
	manualset3
254658	3	425839	7	NULL	NULL	NULL	NULL	CBV5	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coxsackievirus A2 ( CAV2 ) , CBV2 , CBV5 , E7 , E11 , E19 , E24 , E29 and enterovirus 71 were recovered only from sporadic cases .
	manualset3
254660	4	425839	7	NULL	NULL	NULL	NULL	E7	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coxsackievirus A2 ( CAV2 ) , CBV2 , CBV5 , E7 , E11 , E19 , E24 , E29 and enterovirus 71 were recovered only from sporadic cases .
	manualset3
254662	5	425839	7	NULL	NULL	NULL	NULL	E11	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coxsackievirus A2 ( CAV2 ) , CBV2 , CBV5 , E7 , E11 , E19 , E24 , E29 and enterovirus 71 were recovered only from sporadic cases .
	manualset3
254663	6	425839	7	NULL	NULL	NULL	NULL	E19	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coxsackievirus A2 ( CAV2 ) , CBV2 , CBV5 , E7 , E11 , E19 , E24 , E29 and enterovirus 71 were recovered only from sporadic cases .
	manualset3
254664	7	425839	7	NULL	NULL	NULL	NULL	E24	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coxsackievirus A2 ( CAV2 ) , CBV2 , CBV5 , E7 , E11 , E19 , E24 , E29 and enterovirus 71 were recovered only from sporadic cases .
	manualset3
254666	8	425839	7	NULL	NULL	NULL	NULL	E29	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coxsackievirus A2 ( CAV2 ) , CBV2 , CBV5 , E7 , E11 , E19 , E24 , E29 and enterovirus 71 were recovered only from sporadic cases .
	manualset3
254668	9	425839	7	NULL	NULL	NULL	NULL	enterovirus 71	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coxsackievirus A2 ( CAV2 ) , CBV2 , CBV5 , E7 , E11 , E19 , E24 , E29 and enterovirus 71 were recovered only from sporadic cases .
	manualset3
254669	10	425839	7	NULL	NULL	NULL	NULL	sporadic cases	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coxsackievirus A2 ( CAV2 ) , CBV2 , CBV5 , E7 , E11 , E19 , E24 , E29 and enterovirus 71 were recovered only from sporadic cases .
	manualset3
254670	1	425840	7	NULL	NULL	NULL	NULL	Coxsackievirus B3 infection 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coxsackievirus B3 infection in pregnant mice leads to a severe pancreatitis with a retardation of foetal growth and increased wastage .
	manualset3
254671	2	425840	7	NULL	NULL	NULL	NULL	pregnant mice	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coxsackievirus B3 infection in pregnant mice leads to a severe pancreatitis with a retardation of foetal growth and increased wastage .
	manualset3
254672	3	425840	7	NULL	NULL	NULL	NULL	severe pancreatitis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coxsackievirus B3 infection in pregnant mice leads to a severe pancreatitis with a retardation of foetal growth and increased wastage .
	manualset3
254673	4	425840	7	NULL	NULL	NULL	NULL	retardation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coxsackievirus B3 infection in pregnant mice leads to a severe pancreatitis with a retardation of foetal growth and increased wastage .
	manualset3
254674	5	425840	7	NULL	NULL	NULL	NULL	 foetal growth	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coxsackievirus B3 infection in pregnant mice leads to a severe pancreatitis with a retardation of foetal growth and increased wastage .
	manualset3
254675	6	425840	7	NULL	NULL	NULL	NULL	wastage	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Coxsackievirus B3 infection in pregnant mice leads to a severe pancreatitis with a retardation of foetal growth and increased wastage .
	manualset3
254676	1	425841	7	NULL	NULL	NULL	NULL	Cracks	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cracks in the cuticle appeared after cutin synthesis ceased while the seed continued to grow .
	manualset3
254677	2	425841	7	NULL	NULL	NULL	NULL	 cuticle	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cracks in the cuticle appeared after cutin synthesis ceased while the seed continued to grow .
	manualset3
254678	3	425841	7	NULL	NULL	NULL	NULL	cutin synthesis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cracks in the cuticle appeared after cutin synthesis ceased while the seed continued to grow .
	manualset3
254679	4	425841	7	NULL	NULL	NULL	NULL	seed	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cracks in the cuticle appeared after cutin synthesis ceased while the seed continued to grow .
	manualset3
254680	1	425842	7	NULL	NULL	NULL	NULL	Cranial motor neurons	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cranial motor neurons contain either galanin - or calcitonin gene-related peptidelike immunoreactivity .
	manualset3
254681	2	425842	7	NULL	NULL	NULL	NULL	galanin -related peptidelike immunoreactivity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cranial motor neurons contain either galanin - or calcitonin gene-related peptidelike immunoreactivity .
	manualset3
254682	3	425842	7	NULL	NULL	NULL	NULL	calcitonin gene-related peptidelike immunoreactivity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cranial motor neurons contain either galanin - or calcitonin gene-related peptidelike immunoreactivity .
	manualset3
254683	1	425843	7	NULL	NULL	NULL	NULL	Creative Leaders	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Creative Leaders : they generate the magic that best results .
	manualset3
254684	2	425843	7	NULL	NULL	NULL	NULL	magic	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Creative Leaders : they generate the magic that best results .
	manualset3
258598	3	425843	7	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Creative Leaders : they generate the magic that best results .
	manualset3
254693	1	425844	7	NULL	NULL	NULL	NULL	Mast cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Mast cells , histamine and development of the placental vascular network in pregnancies complicated by preeclampsia and intrauterine growth retardation ) .
	manualset3
254694	2	425844	7	NULL	NULL	NULL	NULL	histamine 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Mast cells , histamine and development of the placental vascular network in pregnancies complicated by preeclampsia and intrauterine growth retardation ) .
	manualset3
254695	3	425844	7	NULL	NULL	NULL	NULL	development	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Mast cells , histamine and development of the placental vascular network in pregnancies complicated by preeclampsia and intrauterine growth retardation ) .
	manualset3
254696	4	425844	7	NULL	NULL	NULL	NULL	placental vascular network	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Mast cells , histamine and development of the placental vascular network in pregnancies complicated by preeclampsia and intrauterine growth retardation ) .
	manualset3
254697	5	425844	7	NULL	NULL	NULL	NULL	pregnancies	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Mast cells , histamine and development of the placental vascular network in pregnancies complicated by preeclampsia and intrauterine growth retardation ) .
	manualset3
254698	6	425844	7	NULL	NULL	NULL	NULL	preeclampsia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Mast cells , histamine and development of the placental vascular network in pregnancies complicated by preeclampsia and intrauterine growth retardation ) .
	manualset3
254699	7	425844	7	NULL	NULL	NULL	NULL	 intrauterine growth retardation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Mast cells , histamine and development of the placental vascular network in pregnancies complicated by preeclampsia and intrauterine growth retardation ) .
	manualset3
254700	1	425845	7	NULL	NULL	NULL	NULL	Critical mitral stenosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Critical mitral stenosis was defined by a valve area of less than or equal to 1 cm2 .
	manualset3
254701	2	425845	7	NULL	NULL	NULL	NULL	valve area	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Critical mitral stenosis was defined by a valve area of less than or equal to 1 cm2 .
	manualset3
254702	3	425845	7	NULL	NULL	NULL	NULL	1 cm2	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Critical mitral stenosis was defined by a valve area of less than or equal to 1 cm2 .
	manualset3
254703	1	425846	7	NULL	NULL	NULL	NULL	Critical signaling events 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Critical signaling events during the aminoglycoside-induced death of sensory hair cells in vitro .
	manualset3
254704	2	425846	7	NULL	NULL	NULL	NULL	 aminoglycoside-induced death 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Critical signaling events during the aminoglycoside-induced death of sensory hair cells in vitro .
	manualset3
254705	3	425846	7	NULL	NULL	NULL	NULL	sensory hair cells 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Critical signaling events during the aminoglycoside-induced death of sensory hair cells in vitro .
	manualset3
254706	1	425847	7	NULL	NULL	NULL	NULL	Critical theory	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Critical theory was the perspective used in this analysis and proposal of public health actions to attain social justice .
	manualset3
254707	2	425847	7	NULL	NULL	NULL	NULL	analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Critical theory was the perspective used in this analysis and proposal of public health actions to attain social justice .
	manualset3
254708	3	425847	7	NULL	NULL	NULL	NULL	proposal	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Critical theory was the perspective used in this analysis and proposal of public health actions to attain social justice .
	manualset3
254709	4	425847	7	NULL	NULL	NULL	NULL	public health actions	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Critical theory was the perspective used in this analysis and proposal of public health actions to attain social justice .
	manualset3
254710	5	425847	7	NULL	NULL	NULL	NULL	social justice	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Critical theory was the perspective used in this analysis and proposal of public health actions to attain social justice .
	manualset3
254712	1	425848	7	NULL	NULL	NULL	NULL	Critically injured patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Critically injured patients are at risk for hypothermia .
	manualset3
254713	2	425848	7	NULL	NULL	NULL	NULL	 risk	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Critically injured patients are at risk for hypothermia .
	manualset3
254715	3	425848	7	NULL	NULL	NULL	NULL	hypothermia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Critically injured patients are at risk for hypothermia .
	manualset3
254717	1	425849	7	NULL	NULL	NULL	NULL	Cross-sectional imaging	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cross-sectional imaging is frequently used in the diagnosis of pancreatic cysts , but there can be overlap in radiographic appearance .
	manualset3
254718	2	425849	7	NULL	NULL	NULL	NULL	 diagnosis 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cross-sectional imaging is frequently used in the diagnosis of pancreatic cysts , but there can be overlap in radiographic appearance .
	manualset3
254720	3	425849	7	NULL	NULL	NULL	NULL	pancreatic cysts	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cross-sectional imaging is frequently used in the diagnosis of pancreatic cysts , but there can be overlap in radiographic appearance .
	manualset3
254722	4	425849	7	NULL	NULL	NULL	NULL	overlap	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cross-sectional imaging is frequently used in the diagnosis of pancreatic cysts , but there can be overlap in radiographic appearance .
	manualset3
254724	5	425849	7	NULL	NULL	NULL	NULL	radiographic appearance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cross-sectional imaging is frequently used in the diagnosis of pancreatic cysts , but there can be overlap in radiographic appearance .
	manualset3
254866	1	425850	7	NULL	NULL	NULL	NULL	Cross-sectional surveys	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cross-sectional surveys are unreliable measures of diarrhea prevalence .
	manualset3
254868	2	425850	7	NULL	NULL	NULL	NULL	measures	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cross-sectional surveys are unreliable measures of diarrhea prevalence .
	manualset3
254872	3	425850	7	NULL	NULL	NULL	NULL	diarrhea	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cross-sectional surveys are unreliable measures of diarrhea prevalence .
	manualset3
254883	1	425851	7	NULL	NULL	NULL	NULL	Cross-validation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cross-validation of the Halstead-Reitan tests for brain damage .
	manualset3
254884	2	425851	7	NULL	NULL	NULL	NULL	Halstead-Reitan tests	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cross-validation of the Halstead-Reitan tests for brain damage .
	manualset3
254885	3	425851	7	NULL	NULL	NULL	NULL	brain damage	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cross-validation of the Halstead-Reitan tests for brain damage .
	manualset3
254886	1	425852	7	NULL	NULL	NULL	NULL	Crosstalk	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crosstalk between estrogen receptor and growth factor receptor pathways as a cause for endocrine therapy resistance in breast cancer .
	manualset3
254887	2	425852	7	NULL	NULL	NULL	NULL	estrogen receptor pathways	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crosstalk between estrogen receptor and growth factor receptor pathways as a cause for endocrine therapy resistance in breast cancer .
	manualset3
254892	3	425852	7	NULL	NULL	NULL	NULL	growth factor receptor pathways	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crosstalk between estrogen receptor and growth factor receptor pathways as a cause for endocrine therapy resistance in breast cancer .
	manualset3
254893	4	425852	7	NULL	NULL	NULL	NULL	cause	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crosstalk between estrogen receptor and growth factor receptor pathways as a cause for endocrine therapy resistance in breast cancer .
	manualset3
254894	5	425852	7	NULL	NULL	NULL	NULL	 endocrine therapy resistance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crosstalk between estrogen receptor and growth factor receptor pathways as a cause for endocrine therapy resistance in breast cancer .
	manualset3
254895	6	425852	7	NULL	NULL	NULL	NULL	breast cancer	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crosstalk between estrogen receptor and growth factor receptor pathways as a cause for endocrine therapy resistance in breast cancer .
	manualset3
254896	1	425853	7	NULL	NULL	NULL	NULL	Crowding	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crowding was also affected by an anisotropy based on the target-fixation axis ( radial , tangential , and diagonal ) and by the flankers ' relations .
	manualset3
254897	2	425853	7	NULL	NULL	NULL	NULL	anisotropy	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crowding was also affected by an anisotropy based on the target-fixation axis ( radial , tangential , and diagonal ) and by the flankers ' relations .
	manualset3
254900	3	425853	7	NULL	NULL	NULL	NULL	target-fixation axis	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crowding was also affected by an anisotropy based on the target-fixation axis ( radial , tangential , and diagonal ) and by the flankers ' relations .
	manualset3
254911	4	425853	7	NULL	NULL	NULL	NULL	 flankers ' relations	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crowding was also affected by an anisotropy based on the target-fixation axis ( radial , tangential , and diagonal ) and by the flankers ' relations .
	manualset3
254912	1	425854	7	NULL	NULL	NULL	NULL	Crown fracture	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crown fracture with pulp exposure in primary incisors is a rare condition .
	manualset3
254913	2	425854	7	NULL	NULL	NULL	NULL	pulp exposure	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crown fracture with pulp exposure in primary incisors is a rare condition .
	manualset3
254914	3	425854	7	NULL	NULL	NULL	NULL	primary incisors	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crown fracture with pulp exposure in primary incisors is a rare condition .
	manualset3
254915	4	425854	7	NULL	NULL	NULL	NULL	rare condition	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crown fracture with pulp exposure in primary incisors is a rare condition .
	manualset3
254916	1	425855	7	NULL	NULL	NULL	NULL	Crude decoction	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crude decoction is the most active followed by ethanolic , aqueous and chloroformic extracts in dose-dependent manner and can partly justify the use of the plant in traditional medicine .
	manualset3
254917	2	425855	7	NULL	NULL	NULL	NULL	ethanolic extracts	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crude decoction is the most active followed by ethanolic , aqueous and chloroformic extracts in dose-dependent manner and can partly justify the use of the plant in traditional medicine .
	manualset3
254918	3	425855	7	NULL	NULL	NULL	NULL	 aqueous extracts	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crude decoction is the most active followed by ethanolic , aqueous and chloroformic extracts in dose-dependent manner and can partly justify the use of the plant in traditional medicine .
	manualset3
254919	4	425855	7	NULL	NULL	NULL	NULL	chloroformic extracts 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crude decoction is the most active followed by ethanolic , aqueous and chloroformic extracts in dose-dependent manner and can partly justify the use of the plant in traditional medicine .
	manualset3
254920	5	425855	7	NULL	NULL	NULL	NULL	dose-dependent manner	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crude decoction is the most active followed by ethanolic , aqueous and chloroformic extracts in dose-dependent manner and can partly justify the use of the plant in traditional medicine .
	manualset3
254921	6	425855	7	NULL	NULL	NULL	NULL	use	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crude decoction is the most active followed by ethanolic , aqueous and chloroformic extracts in dose-dependent manner and can partly justify the use of the plant in traditional medicine .
	manualset3
254922	7	425855	7	NULL	NULL	NULL	NULL	plant	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crude decoction is the most active followed by ethanolic , aqueous and chloroformic extracts in dose-dependent manner and can partly justify the use of the plant in traditional medicine .
	manualset3
254923	8	425855	7	NULL	NULL	NULL	NULL	traditional medicine	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crude decoction is the most active followed by ethanolic , aqueous and chloroformic extracts in dose-dependent manner and can partly justify the use of the plant in traditional medicine .
	manualset3
254934	1	425856	7	NULL	NULL	NULL	NULL	Cryoablation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cryoablation versus radiofrequency ablation for atrioventricular nodal reentrant tachycardia : patient pain perception and operator stress .
	manualset3
254935	2	425856	7	NULL	NULL	NULL	NULL	radiofrequency ablation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cryoablation versus radiofrequency ablation for atrioventricular nodal reentrant tachycardia : patient pain perception and operator stress .
	manualset3
254936	3	425856	7	NULL	NULL	NULL	NULL	atrioventricular nodal reentrant tachycardia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cryoablation versus radiofrequency ablation for atrioventricular nodal reentrant tachycardia : patient pain perception and operator stress .
	manualset3
254937	4	425856	7	NULL	NULL	NULL	NULL	 patient pain perception	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cryoablation versus radiofrequency ablation for atrioventricular nodal reentrant tachycardia : patient pain perception and operator stress .
	manualset3
254938	5	425856	7	NULL	NULL	NULL	NULL	operator stress	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cryoablation versus radiofrequency ablation for atrioventricular nodal reentrant tachycardia : patient pain perception and operator stress .
	manualset3
254939	1	425857	7	NULL	NULL	NULL	NULL	Measurement	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Measurement of alpha-fetoprotein with L3 fraction in the early diagnosis of patients with hepatocellular carcinoma ) .
	manualset3
254940	2	425857	7	NULL	NULL	NULL	NULL	alpha-fetoprotein	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Measurement of alpha-fetoprotein with L3 fraction in the early diagnosis of patients with hepatocellular carcinoma ) .
	manualset3
254941	3	425857	7	NULL	NULL	NULL	NULL	L3 fraction	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Measurement of alpha-fetoprotein with L3 fraction in the early diagnosis of patients with hepatocellular carcinoma ) .
	manualset3
254942	4	425857	7	NULL	NULL	NULL	NULL	early diagnosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Measurement of alpha-fetoprotein with L3 fraction in the early diagnosis of patients with hepatocellular carcinoma ) .
	manualset3
254943	5	425857	7	NULL	NULL	NULL	NULL	 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Measurement of alpha-fetoprotein with L3 fraction in the early diagnosis of patients with hepatocellular carcinoma ) .
	manualset3
254944	6	425857	7	NULL	NULL	NULL	NULL	 hepatocellular carcinoma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Measurement of alpha-fetoprotein with L3 fraction in the early diagnosis of patients with hepatocellular carcinoma ) .
	manualset3
254945	1	425858	7	NULL	NULL	NULL	NULL	Cryostat sections	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cryostat sections are used from brain or extracerebral tissue in dog , monkey , rat and mouse and exposed for 3 s to a room temperature solution containing sucrose-potassium phosphate-glyoxylic acid ( SPG ) .
	manualset3
254946	2	425858	7	NULL	NULL	NULL	NULL	brain	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cryostat sections are used from brain or extracerebral tissue in dog , monkey , rat and mouse and exposed for 3 s to a room temperature solution containing sucrose-potassium phosphate-glyoxylic acid ( SPG ) .
	manualset3
254947	3	425858	7	NULL	NULL	NULL	NULL	extracerebral tissue	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cryostat sections are used from brain or extracerebral tissue in dog , monkey , rat and mouse and exposed for 3 s to a room temperature solution containing sucrose-potassium phosphate-glyoxylic acid ( SPG ) .
	manualset3
254948	4	425858	7	NULL	NULL	NULL	NULL	 dog	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cryostat sections are used from brain or extracerebral tissue in dog , monkey , rat and mouse and exposed for 3 s to a room temperature solution containing sucrose-potassium phosphate-glyoxylic acid ( SPG ) .
	manualset3
254949	5	425858	7	NULL	NULL	NULL	NULL	monkey	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cryostat sections are used from brain or extracerebral tissue in dog , monkey , rat and mouse and exposed for 3 s to a room temperature solution containing sucrose-potassium phosphate-glyoxylic acid ( SPG ) .
	manualset3
254950	6	425858	7	NULL	NULL	NULL	NULL	 rat	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cryostat sections are used from brain or extracerebral tissue in dog , monkey , rat and mouse and exposed for 3 s to a room temperature solution containing sucrose-potassium phosphate-glyoxylic acid ( SPG ) .
	manualset3
254952	7	425858	7	NULL	NULL	NULL	NULL	mouse	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cryostat sections are used from brain or extracerebral tissue in dog , monkey , rat and mouse and exposed for 3 s to a room temperature solution containing sucrose-potassium phosphate-glyoxylic acid ( SPG ) .
	manualset3
254955	8	425858	7	NULL	NULL	NULL	NULL	3 s	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cryostat sections are used from brain or extracerebral tissue in dog , monkey , rat and mouse and exposed for 3 s to a room temperature solution containing sucrose-potassium phosphate-glyoxylic acid ( SPG ) .
	manualset3
254958	9	425858	7	NULL	NULL	NULL	NULL	 room temperature solution 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cryostat sections are used from brain or extracerebral tissue in dog , monkey , rat and mouse and exposed for 3 s to a room temperature solution containing sucrose-potassium phosphate-glyoxylic acid ( SPG ) .
	manualset3
254960	10	425858	7	NULL	NULL	NULL	NULL	sucrose-potassium phosphate-glyoxylic acid ( SPG ) 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cryostat sections are used from brain or extracerebral tissue in dog , monkey , rat and mouse and exposed for 3 s to a room temperature solution containing sucrose-potassium phosphate-glyoxylic acid ( SPG ) .
	manualset3
254965	1	425859	7	NULL	NULL	NULL	NULL	Cryptosporidium	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cryptosporidium in water : CDC guidelines on how to protect yourself .
	manualset3
254967	2	425859	7	NULL	NULL	NULL	NULL	water	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cryptosporidium in water : CDC guidelines on how to protect yourself .
	manualset3
254969	3	425859	7	NULL	NULL	NULL	NULL	CDC guidelines	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cryptosporidium in water : CDC guidelines on how to protect yourself .
	manualset3
254972	1	425860	7	NULL	NULL	NULL	NULL	Crystal engineering 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystal engineering of metalloporphyrin assemblies .
	manualset3
254975	2	425860	7	NULL	NULL	NULL	NULL	 metalloporphyrin assemblies	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystal engineering of metalloporphyrin assemblies .
	manualset3
254985	1	425861	7	NULL	NULL	NULL	NULL	Crystal induced inflammation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystal induced inflammation in canine joints .
	manualset3
254986	2	425861	7	NULL	NULL	NULL	NULL	canine joints	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystal induced inflammation in canine joints .
	manualset3
254987	1	425862	7	NULL	NULL	NULL	NULL	Crystal structure	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystal structure and thermodynamic analysis of human brain fatty acid-binding protein .
	manualset3
254988	2	425862	7	NULL	NULL	NULL	NULL	thermodynamic analysis	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystal structure and thermodynamic analysis of human brain fatty acid-binding protein .
	manualset3
254989	3	425862	7	NULL	NULL	NULL	NULL	human brain fatty acid-binding protein	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystal structure and thermodynamic analysis of human brain fatty acid-binding protein .
	manualset3
254990	1	425863	7	NULL	NULL	NULL	NULL	Crystal structures	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystal structures have been determined of complexes between a 22-mer intramolecular human telomeric quadruplex and two potent tetra-substituted naphthalene diimide compounds , functionalized with positively charged N-methyl-piperazine side-chains .
	manualset3
254992	2	425863	7	NULL	NULL	NULL	NULL	complexes	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystal structures have been determined of complexes between a 22-mer intramolecular human telomeric quadruplex and two potent tetra-substituted naphthalene diimide compounds , functionalized with positively charged N-methyl-piperazine side-chains .
	manualset3
254995	3	425863	7	NULL	NULL	NULL	NULL	22-mer intramolecular human telomeric quadruplex	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystal structures have been determined of complexes between a 22-mer intramolecular human telomeric quadruplex and two potent tetra-substituted naphthalene diimide compounds , functionalized with positively charged N-methyl-piperazine side-chains .
	manualset3
254996	4	425863	7	NULL	NULL	NULL	NULL	two potent tetra-substituted naphthalene diimide compounds	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystal structures have been determined of complexes between a 22-mer intramolecular human telomeric quadruplex and two potent tetra-substituted naphthalene diimide compounds , functionalized with positively charged N-methyl-piperazine side-chains .
	manualset3
254999	5	425863	7	NULL	NULL	NULL	NULL	 positively charged N-methyl-piperazine side-chains	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystal structures have been determined of complexes between a 22-mer intramolecular human telomeric quadruplex and two potent tetra-substituted naphthalene diimide compounds , functionalized with positively charged N-methyl-piperazine side-chains .
	manualset3
255057	1	425864	7	NULL	NULL	NULL	NULL	Crystal structures 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystal structures of the ligand-free antibody fragments showed no noteworthy conformational changes due to humanization , and the loop structures of the CDRs of the humanized antibodies were identical to those of the parent antibodies .
	manualset3
255058	2	425864	7	NULL	NULL	NULL	NULL	ligand-free antibody fragments	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystal structures of the ligand-free antibody fragments showed no noteworthy conformational changes due to humanization , and the loop structures of the CDRs of the humanized antibodies were identical to those of the parent antibodies .
	manualset3
255059	3	425864	7	NULL	NULL	NULL	NULL	conformational changes	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystal structures of the ligand-free antibody fragments showed no noteworthy conformational changes due to humanization , and the loop structures of the CDRs of the humanized antibodies were identical to those of the parent antibodies .
	manualset3
255060	4	425864	7	NULL	NULL	NULL	NULL	humanization	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystal structures of the ligand-free antibody fragments showed no noteworthy conformational changes due to humanization , and the loop structures of the CDRs of the humanized antibodies were identical to those of the parent antibodies .
	manualset3
255061	5	425864	7	NULL	NULL	NULL	NULL	loop structures	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystal structures of the ligand-free antibody fragments showed no noteworthy conformational changes due to humanization , and the loop structures of the CDRs of the humanized antibodies were identical to those of the parent antibodies .
	manualset3
255062	6	425864	7	NULL	NULL	NULL	NULL	 CDRs	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystal structures of the ligand-free antibody fragments showed no noteworthy conformational changes due to humanization , and the loop structures of the CDRs of the humanized antibodies were identical to those of the parent antibodies .
	manualset3
255063	7	425864	7	NULL	NULL	NULL	NULL	humanized antibodies 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystal structures of the ligand-free antibody fragments showed no noteworthy conformational changes due to humanization , and the loop structures of the CDRs of the humanized antibodies were identical to those of the parent antibodies .
	manualset3
255064	8	425864	7	NULL	NULL	NULL	NULL	parent antibodies	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystal structures of the ligand-free antibody fragments showed no noteworthy conformational changes due to humanization , and the loop structures of the CDRs of the humanized antibodies were identical to those of the parent antibodies .
	manualset3
255065	1	425865	7	NULL	NULL	NULL	NULL	Crystalline biominerals	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystalline or amorphous biominerals , an important category of mineralogical biosignatures , precipitate under direct cellular control as part of the life cycle of the organism ( shells , tests , phytoliths ) or indirectly when cell surface layers provide sites for heterogeneous nucleation .
	manualset3
255066	2	425865	7	NULL	NULL	NULL	NULL	amorphous biominerals	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystalline or amorphous biominerals , an important category of mineralogical biosignatures , precipitate under direct cellular control as part of the life cycle of the organism ( shells , tests , phytoliths ) or indirectly when cell surface layers provide sites for heterogeneous nucleation .
	manualset3
255067	3	425865	7	NULL	NULL	NULL	NULL	 category	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystalline or amorphous biominerals , an important category of mineralogical biosignatures , precipitate under direct cellular control as part of the life cycle of the organism ( shells , tests , phytoliths ) or indirectly when cell surface layers provide sites for heterogeneous nucleation .
	manualset3
255068	4	425865	7	NULL	NULL	NULL	NULL	mineralogical biosignatures	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystalline or amorphous biominerals , an important category of mineralogical biosignatures , precipitate under direct cellular control as part of the life cycle of the organism ( shells , tests , phytoliths ) or indirectly when cell surface layers provide sites for heterogeneous nucleation .
	manualset3
255069	5	425865	7	NULL	NULL	NULL	NULL	direct cellular control	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystalline or amorphous biominerals , an important category of mineralogical biosignatures , precipitate under direct cellular control as part of the life cycle of the organism ( shells , tests , phytoliths ) or indirectly when cell surface layers provide sites for heterogeneous nucleation .
	manualset3
255070	6	425865	7	NULL	NULL	NULL	NULL	 part of the life cycle	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystalline or amorphous biominerals , an important category of mineralogical biosignatures , precipitate under direct cellular control as part of the life cycle of the organism ( shells , tests , phytoliths ) or indirectly when cell surface layers provide sites for heterogeneous nucleation .
	manualset3
255071	7	425865	7	NULL	NULL	NULL	NULL	organism	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystalline or amorphous biominerals , an important category of mineralogical biosignatures , precipitate under direct cellular control as part of the life cycle of the organism ( shells , tests , phytoliths ) or indirectly when cell surface layers provide sites for heterogeneous nucleation .
	manualset3
255072	8	425865	7	NULL	NULL	NULL	NULL	shells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystalline or amorphous biominerals , an important category of mineralogical biosignatures , precipitate under direct cellular control as part of the life cycle of the organism ( shells , tests , phytoliths ) or indirectly when cell surface layers provide sites for heterogeneous nucleation .
	manualset3
255073	9	425865	7	NULL	NULL	NULL	NULL	 tests	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystalline or amorphous biominerals , an important category of mineralogical biosignatures , precipitate under direct cellular control as part of the life cycle of the organism ( shells , tests , phytoliths ) or indirectly when cell surface layers provide sites for heterogeneous nucleation .
	manualset3
255074	10	425865	7	NULL	NULL	NULL	NULL	phytoliths 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystalline or amorphous biominerals , an important category of mineralogical biosignatures , precipitate under direct cellular control as part of the life cycle of the organism ( shells , tests , phytoliths ) or indirectly when cell surface layers provide sites for heterogeneous nucleation .
	manualset3
255075	11	425865	7	NULL	NULL	NULL	NULL	cell surface layers	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystalline or amorphous biominerals , an important category of mineralogical biosignatures , precipitate under direct cellular control as part of the life cycle of the organism ( shells , tests , phytoliths ) or indirectly when cell surface layers provide sites for heterogeneous nucleation .
	manualset3
255076	12	425865	7	NULL	NULL	NULL	NULL	 sites 	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystalline or amorphous biominerals , an important category of mineralogical biosignatures , precipitate under direct cellular control as part of the life cycle of the organism ( shells , tests , phytoliths ) or indirectly when cell surface layers provide sites for heterogeneous nucleation .
	manualset3
255077	13	425865	7	NULL	NULL	NULL	NULL	heterogeneous nucleation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystalline or amorphous biominerals , an important category of mineralogical biosignatures , precipitate under direct cellular control as part of the life cycle of the organism ( shells , tests , phytoliths ) or indirectly when cell surface layers provide sites for heterogeneous nucleation .
	manualset3
255078	1	425866	7	NULL	NULL	NULL	NULL	Crystallization 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystallization and preliminary X-ray diffraction analysis of a type I beta-glucosidase encoded by the bgIA gene of Bacillus polymyxa .
	manualset3
255079	2	425866	7	NULL	NULL	NULL	NULL	X-ray diffraction analysis	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystallization and preliminary X-ray diffraction analysis of a type I beta-glucosidase encoded by the bgIA gene of Bacillus polymyxa .
	manualset3
255080	3	425866	7	NULL	NULL	NULL	NULL	 type I beta-glucosidase	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystallization and preliminary X-ray diffraction analysis of a type I beta-glucosidase encoded by the bgIA gene of Bacillus polymyxa .
	manualset3
255081	4	425866	7	NULL	NULL	NULL	NULL	bgIA gene	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystallization and preliminary X-ray diffraction analysis of a type I beta-glucosidase encoded by the bgIA gene of Bacillus polymyxa .
	manualset3
255082	5	425866	7	NULL	NULL	NULL	NULL	Bacillus polymyxa	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystallization and preliminary X-ray diffraction analysis of a type I beta-glucosidase encoded by the bgIA gene of Bacillus polymyxa .
	manualset3
255083	1	425867	7	NULL	NULL	NULL	NULL	Mechanism 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Mechanism of action of certain fibrinolytic bis-tetrahydroisoquinolines : their antagonists and histamine - and 5-hydroxytryptamine-releasing effects ( author 's transl ) ) .
	manualset3
255084	2	425867	7	NULL	NULL	NULL	NULL	action	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Mechanism of action of certain fibrinolytic bis-tetrahydroisoquinolines : their antagonists and histamine - and 5-hydroxytryptamine-releasing effects ( author 's transl ) ) .
	manualset3
255085	3	425867	7	NULL	NULL	NULL	NULL	fibrinolytic bis-tetrahydroisoquinolines	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Mechanism of action of certain fibrinolytic bis-tetrahydroisoquinolines : their antagonists and histamine - and 5-hydroxytryptamine-releasing effects ( author 's transl ) ) .
	manualset3
255086	4	425867	7	NULL	NULL	NULL	NULL	antagonists	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Mechanism of action of certain fibrinolytic bis-tetrahydroisoquinolines : their antagonists and histamine - and 5-hydroxytryptamine-releasing effects ( author 's transl ) ) .
	manualset3
255087	5	425867	7	NULL	NULL	NULL	NULL	histamine 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Mechanism of action of certain fibrinolytic bis-tetrahydroisoquinolines : their antagonists and histamine - and 5-hydroxytryptamine-releasing effects ( author 's transl ) ) .
	manualset3
255088	6	425867	7	NULL	NULL	NULL	NULL	5-hydroxytryptamine-releasing effects	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Mechanism of action of certain fibrinolytic bis-tetrahydroisoquinolines : their antagonists and histamine - and 5-hydroxytryptamine-releasing effects ( author 's transl ) ) .
	manualset3
255089	7	425867	7	NULL	NULL	NULL	NULL	author 's transl 	PublicationOrCitation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Mechanism of action of certain fibrinolytic bis-tetrahydroisoquinolines : their antagonists and histamine - and 5-hydroxytryptamine-releasing effects ( author 's transl ) ) .
	manualset3
255090	1	425868	7	NULL	NULL	NULL	NULL	Crystalloids	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystalloids are the preferred fluids , while colloids may be used in some situations .
	manualset3
255091	2	425868	7	NULL	NULL	NULL	NULL	 fluids	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystalloids are the preferred fluids , while colloids may be used in some situations .
	manualset3
255092	3	425868	7	NULL	NULL	NULL	NULL	 colloids	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystalloids are the preferred fluids , while colloids may be used in some situations .
	manualset3
255093	4	425868	7	NULL	NULL	NULL	NULL	 situations	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystalloids are the preferred fluids , while colloids may be used in some situations .
	manualset3
255094	1	425869	7	NULL	NULL	NULL	NULL	Crystals	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystals of the 1 , 2-dichloroethane hemisolvate of TpWOS ( S ( 2 ) PPh ( 2 ) - S ) belong to the triclinic space group Ponemacr ; with a = 10.732 ( 6 ) A , b = 16.91 ( 1 ) A , c = 10.021 ( 4 ) A , alpha = 104.40 ( 4 ) degrees , beta = 107.52 ( 3 ) degrees , gamma = 96.09 ( 5 ) degrees , V = 1647 ( 1 ) A ( 3 ) for Z = 2 .
	manualset3
255095	2	425869	7	NULL	NULL	NULL	NULL	 1 , 2-dichloroethane hemisolvate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystals of the 1 , 2-dichloroethane hemisolvate of TpWOS ( S ( 2 ) PPh ( 2 ) - S ) belong to the triclinic space group Ponemacr ; with a = 10.732 ( 6 ) A , b = 16.91 ( 1 ) A , c = 10.021 ( 4 ) A , alpha = 104.40 ( 4 ) degrees , beta = 107.52 ( 3 ) degrees , gamma = 96.09 ( 5 ) degrees , V = 1647 ( 1 ) A ( 3 ) for Z = 2 .
	manualset3
255096	3	425869	7	NULL	NULL	NULL	NULL	TpWOS ( S ( 2 ) PPh ( 2 ) - S )	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystals of the 1 , 2-dichloroethane hemisolvate of TpWOS ( S ( 2 ) PPh ( 2 ) - S ) belong to the triclinic space group Ponemacr ; with a = 10.732 ( 6 ) A , b = 16.91 ( 1 ) A , c = 10.021 ( 4 ) A , alpha = 104.40 ( 4 ) degrees , beta = 107.52 ( 3 ) degrees , gamma = 96.09 ( 5 ) degrees , V = 1647 ( 1 ) A ( 3 ) for Z = 2 .
	manualset3
255097	4	425869	7	NULL	NULL	NULL	NULL	triclinic space group	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystals of the 1 , 2-dichloroethane hemisolvate of TpWOS ( S ( 2 ) PPh ( 2 ) - S ) belong to the triclinic space group Ponemacr ; with a = 10.732 ( 6 ) A , b = 16.91 ( 1 ) A , c = 10.021 ( 4 ) A , alpha = 104.40 ( 4 ) degrees , beta = 107.52 ( 3 ) degrees , gamma = 96.09 ( 5 ) degrees , V = 1647 ( 1 ) A ( 3 ) for Z = 2 .
	manualset3
255098	5	425869	7	NULL	NULL	NULL	NULL	Ponemacr	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystals of the 1 , 2-dichloroethane hemisolvate of TpWOS ( S ( 2 ) PPh ( 2 ) - S ) belong to the triclinic space group Ponemacr ; with a = 10.732 ( 6 ) A , b = 16.91 ( 1 ) A , c = 10.021 ( 4 ) A , alpha = 104.40 ( 4 ) degrees , beta = 107.52 ( 3 ) degrees , gamma = 96.09 ( 5 ) degrees , V = 1647 ( 1 ) A ( 3 ) for Z = 2 .
	manualset3
255099	6	425869	7	NULL	NULL	NULL	NULL	a = 10.732 ( 6 ) A	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystals of the 1 , 2-dichloroethane hemisolvate of TpWOS ( S ( 2 ) PPh ( 2 ) - S ) belong to the triclinic space group Ponemacr ; with a = 10.732 ( 6 ) A , b = 16.91 ( 1 ) A , c = 10.021 ( 4 ) A , alpha = 104.40 ( 4 ) degrees , beta = 107.52 ( 3 ) degrees , gamma = 96.09 ( 5 ) degrees , V = 1647 ( 1 ) A ( 3 ) for Z = 2 .
	manualset3
255100	7	425869	7	NULL	NULL	NULL	NULL	b = 16.91 ( 1 ) A 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystals of the 1 , 2-dichloroethane hemisolvate of TpWOS ( S ( 2 ) PPh ( 2 ) - S ) belong to the triclinic space group Ponemacr ; with a = 10.732 ( 6 ) A , b = 16.91 ( 1 ) A , c = 10.021 ( 4 ) A , alpha = 104.40 ( 4 ) degrees , beta = 107.52 ( 3 ) degrees , gamma = 96.09 ( 5 ) degrees , V = 1647 ( 1 ) A ( 3 ) for Z = 2 .
	manualset3
255101	8	425869	7	NULL	NULL	NULL	NULL	c = 10.021 ( 4 ) A 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystals of the 1 , 2-dichloroethane hemisolvate of TpWOS ( S ( 2 ) PPh ( 2 ) - S ) belong to the triclinic space group Ponemacr ; with a = 10.732 ( 6 ) A , b = 16.91 ( 1 ) A , c = 10.021 ( 4 ) A , alpha = 104.40 ( 4 ) degrees , beta = 107.52 ( 3 ) degrees , gamma = 96.09 ( 5 ) degrees , V = 1647 ( 1 ) A ( 3 ) for Z = 2 .
	manualset3
255102	9	425869	7	NULL	NULL	NULL	NULL	alpha = 104.40 ( 4 ) degrees	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystals of the 1 , 2-dichloroethane hemisolvate of TpWOS ( S ( 2 ) PPh ( 2 ) - S ) belong to the triclinic space group Ponemacr ; with a = 10.732 ( 6 ) A , b = 16.91 ( 1 ) A , c = 10.021 ( 4 ) A , alpha = 104.40 ( 4 ) degrees , beta = 107.52 ( 3 ) degrees , gamma = 96.09 ( 5 ) degrees , V = 1647 ( 1 ) A ( 3 ) for Z = 2 .
	manualset3
255103	10	425869	7	NULL	NULL	NULL	NULL	beta = 107.52 ( 3 ) degrees	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystals of the 1 , 2-dichloroethane hemisolvate of TpWOS ( S ( 2 ) PPh ( 2 ) - S ) belong to the triclinic space group Ponemacr ; with a = 10.732 ( 6 ) A , b = 16.91 ( 1 ) A , c = 10.021 ( 4 ) A , alpha = 104.40 ( 4 ) degrees , beta = 107.52 ( 3 ) degrees , gamma = 96.09 ( 5 ) degrees , V = 1647 ( 1 ) A ( 3 ) for Z = 2 .
	manualset3
255104	11	425869	7	NULL	NULL	NULL	NULL	gamma = 96.09 ( 5 ) degrees	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystals of the 1 , 2-dichloroethane hemisolvate of TpWOS ( S ( 2 ) PPh ( 2 ) - S ) belong to the triclinic space group Ponemacr ; with a = 10.732 ( 6 ) A , b = 16.91 ( 1 ) A , c = 10.021 ( 4 ) A , alpha = 104.40 ( 4 ) degrees , beta = 107.52 ( 3 ) degrees , gamma = 96.09 ( 5 ) degrees , V = 1647 ( 1 ) A ( 3 ) for Z = 2 .
	manualset3
255105	12	425869	7	NULL	NULL	NULL	NULL	V = 1647 ( 1 ) A ( 3 )	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystals of the 1 , 2-dichloroethane hemisolvate of TpWOS ( S ( 2 ) PPh ( 2 ) - S ) belong to the triclinic space group Ponemacr ; with a = 10.732 ( 6 ) A , b = 16.91 ( 1 ) A , c = 10.021 ( 4 ) A , alpha = 104.40 ( 4 ) degrees , beta = 107.52 ( 3 ) degrees , gamma = 96.09 ( 5 ) degrees , V = 1647 ( 1 ) A ( 3 ) for Z = 2 .
	manualset3
255106	13	425869	7	NULL	NULL	NULL	NULL	Z = 2	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Crystals of the 1 , 2-dichloroethane hemisolvate of TpWOS ( S ( 2 ) PPh ( 2 ) - S ) belong to the triclinic space group Ponemacr ; with a = 10.732 ( 6 ) A , b = 16.91 ( 1 ) A , c = 10.021 ( 4 ) A , alpha = 104.40 ( 4 ) degrees , beta = 107.52 ( 3 ) degrees , gamma = 96.09 ( 5 ) degrees , V = 1647 ( 1 ) A ( 3 ) for Z = 2 .
	manualset3
255107	1	425870	7	NULL	NULL	NULL	NULL	CsA 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	CsA ( 10 mg/kg/d ) suppressed the expression of iNOS in response to balloon-induced aortic injury .
	manualset3
255108	2	425870	7	NULL	NULL	NULL	NULL	10 mg/kg/d	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	CsA ( 10 mg/kg/d ) suppressed the expression of iNOS in response to balloon-induced aortic injury .
	manualset3
255109	3	425870	7	NULL	NULL	NULL	NULL	 expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	CsA ( 10 mg/kg/d ) suppressed the expression of iNOS in response to balloon-induced aortic injury .
	manualset3
255110	4	425870	7	NULL	NULL	NULL	NULL	 iNOS	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	CsA ( 10 mg/kg/d ) suppressed the expression of iNOS in response to balloon-induced aortic injury .
	manualset3
255111	5	425870	7	NULL	NULL	NULL	NULL	 balloon-induced aortic injury	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	CsA ( 10 mg/kg/d ) suppressed the expression of iNOS in response to balloon-induced aortic injury .
	manualset3
255112	1	425871	7	NULL	NULL	NULL	NULL	CspA	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	CspA consists of a five-stranded beta-barrel structure containing two RNA-binding motifs , RNP1 and RNP2 .
	manualset3
255113	2	425871	7	NULL	NULL	NULL	NULL	five-stranded beta-barrel structure 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	CspA consists of a five-stranded beta-barrel structure containing two RNA-binding motifs , RNP1 and RNP2 .
	manualset3
255114	3	425871	7	NULL	NULL	NULL	NULL	two RNA-binding motifs	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	CspA consists of a five-stranded beta-barrel structure containing two RNA-binding motifs , RNP1 and RNP2 .
	manualset3
255115	4	425871	7	NULL	NULL	NULL	NULL	RNP1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	CspA consists of a five-stranded beta-barrel structure containing two RNA-binding motifs , RNP1 and RNP2 .
	manualset3
255116	5	425871	7	NULL	NULL	NULL	NULL	RNP2	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	CspA consists of a five-stranded beta-barrel structure containing two RNA-binding motifs , RNP1 and RNP2 .
	manualset3
255117	1	425872	7	NULL	NULL	NULL	NULL	Cu-deficient ( CuD ) Postnatal Day 24 ( P24 ) rats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cu-deficient ( CuD ) Postnatal Day 24 ( P24 ) rats from both experiments demonstrated lower hemoglobin , serum Fe and serum triiodothyronine ( T3 ) concentrations .
	manualset3
255118	2	425872	7	NULL	NULL	NULL	NULL	experiments	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cu-deficient ( CuD ) Postnatal Day 24 ( P24 ) rats from both experiments demonstrated lower hemoglobin , serum Fe and serum triiodothyronine ( T3 ) concentrations .
	manualset3
255119	3	425872	7	NULL	NULL	NULL	NULL	lower hemoglobin	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cu-deficient ( CuD ) Postnatal Day 24 ( P24 ) rats from both experiments demonstrated lower hemoglobin , serum Fe and serum triiodothyronine ( T3 ) concentrations .
	manualset3
255120	4	425872	7	NULL	NULL	NULL	NULL	serum Fe concentration	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cu-deficient ( CuD ) Postnatal Day 24 ( P24 ) rats from both experiments demonstrated lower hemoglobin , serum Fe and serum triiodothyronine ( T3 ) concentrations .
	manualset3
255121	5	425872	7	NULL	NULL	NULL	NULL	serum triiodothyronine ( T3 ) concentrations	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cu-deficient ( CuD ) Postnatal Day 24 ( P24 ) rats from both experiments demonstrated lower hemoglobin , serum Fe and serum triiodothyronine ( T3 ) concentrations .
	manualset3
255848	1	425873	7	NULL	NULL	NULL	NULL	Cubitus varus	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cubitus varus : a new and simple technique for correction .
	manualset3
255849	2	425873	7	NULL	NULL	NULL	NULL	simple technique	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cubitus varus : a new and simple technique for correction .
	manualset3
255850	3	425873	7	NULL	NULL	NULL	NULL	correction	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cubitus varus : a new and simple technique for correction .
	manualset3
255851	1	425874	7	NULL	NULL	NULL	NULL	Cuf2	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cuf2 is a novel meiosis-specific regulatory factor of meiosis maturation .
	manualset3
255852	2	425874	7	NULL	NULL	NULL	NULL	novel meiosis-specific regulatory factor 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cuf2 is a novel meiosis-specific regulatory factor of meiosis maturation .
	manualset3
255853	3	425874	7	NULL	NULL	NULL	NULL	meiosis maturation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cuf2 is a novel meiosis-specific regulatory factor of meiosis maturation .
	manualset3
255854	1	425875	7	NULL	NULL	NULL	NULL	Cultural differences	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultural and ethnic differences , as well as dietary variability , especially in a diseased state have been implicated in the differences observed in the fatty acid composition in peripheral blood mononuclear cell membranes of patients with multiple sclerosis .
	manualset3
255855	2	425875	7	NULL	NULL	NULL	NULL	ethnic differences	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultural and ethnic differences , as well as dietary variability , especially in a diseased state have been implicated in the differences observed in the fatty acid composition in peripheral blood mononuclear cell membranes of patients with multiple sclerosis .
	manualset3
255856	3	425875	7	NULL	NULL	NULL	NULL	dietary variability	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultural and ethnic differences , as well as dietary variability , especially in a diseased state have been implicated in the differences observed in the fatty acid composition in peripheral blood mononuclear cell membranes of patients with multiple sclerosis .
	manualset3
255857	4	425875	7	NULL	NULL	NULL	NULL	diseased state	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultural and ethnic differences , as well as dietary variability , especially in a diseased state have been implicated in the differences observed in the fatty acid composition in peripheral blood mononuclear cell membranes of patients with multiple sclerosis .
	manualset3
255858	5	425875	7	NULL	NULL	NULL	NULL	 differences 	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultural and ethnic differences , as well as dietary variability , especially in a diseased state have been implicated in the differences observed in the fatty acid composition in peripheral blood mononuclear cell membranes of patients with multiple sclerosis .
	manualset3
255859	6	425875	7	NULL	NULL	NULL	NULL	 fatty acid composition 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultural and ethnic differences , as well as dietary variability , especially in a diseased state have been implicated in the differences observed in the fatty acid composition in peripheral blood mononuclear cell membranes of patients with multiple sclerosis .
	manualset3
255860	7	425875	7	NULL	NULL	NULL	NULL	peripheral blood mononuclear cell membranes	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultural and ethnic differences , as well as dietary variability , especially in a diseased state have been implicated in the differences observed in the fatty acid composition in peripheral blood mononuclear cell membranes of patients with multiple sclerosis .
	manualset3
255861	8	425875	7	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultural and ethnic differences , as well as dietary variability , especially in a diseased state have been implicated in the differences observed in the fatty acid composition in peripheral blood mononuclear cell membranes of patients with multiple sclerosis .
	manualset3
255862	9	425875	7	NULL	NULL	NULL	NULL	multiple sclerosis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultural and ethnic differences , as well as dietary variability , especially in a diseased state have been implicated in the differences observed in the fatty acid composition in peripheral blood mononuclear cell membranes of patients with multiple sclerosis .
	manualset3
255863	1	425876	7	NULL	NULL	NULL	NULL	Cultural preferences	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultural preferences for the sex of offspring may produce behavior , such as female infanticide , sex-selective abortion and sex-selective parental investment , which alter the sex ratio in a population .
	manualset3
255864	2	425876	7	NULL	NULL	NULL	NULL	sex	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultural preferences for the sex of offspring may produce behavior , such as female infanticide , sex-selective abortion and sex-selective parental investment , which alter the sex ratio in a population .
	manualset3
255865	3	425876	7	NULL	NULL	NULL	NULL	offspring	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultural preferences for the sex of offspring may produce behavior , such as female infanticide , sex-selective abortion and sex-selective parental investment , which alter the sex ratio in a population .
	manualset3
255866	4	425876	7	NULL	NULL	NULL	NULL	behavior	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultural preferences for the sex of offspring may produce behavior , such as female infanticide , sex-selective abortion and sex-selective parental investment , which alter the sex ratio in a population .
	manualset3
255867	5	425876	7	NULL	NULL	NULL	NULL	 female infanticide	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultural preferences for the sex of offspring may produce behavior , such as female infanticide , sex-selective abortion and sex-selective parental investment , which alter the sex ratio in a population .
	manualset3
255868	6	425876	7	NULL	NULL	NULL	NULL	sex-selective abortion	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultural preferences for the sex of offspring may produce behavior , such as female infanticide , sex-selective abortion and sex-selective parental investment , which alter the sex ratio in a population .
	manualset3
255869	7	425876	7	NULL	NULL	NULL	NULL	sex-selective parental investment 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultural preferences for the sex of offspring may produce behavior , such as female infanticide , sex-selective abortion and sex-selective parental investment , which alter the sex ratio in a population .
	manualset3
255870	8	425876	7	NULL	NULL	NULL	NULL	sex ratio	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultural preferences for the sex of offspring may produce behavior , such as female infanticide , sex-selective abortion and sex-selective parental investment , which alter the sex ratio in a population .
	manualset3
255871	9	425876	7	NULL	NULL	NULL	NULL	population 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultural preferences for the sex of offspring may produce behavior , such as female infanticide , sex-selective abortion and sex-selective parental investment , which alter the sex ratio in a population .
	manualset3
255872	1	425877	7	NULL	NULL	NULL	NULL	Culture-independent analysis	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Culture-independent analysis combined with culture-based methods indicated the presence of thermophilic crenarchaeal and gram-positive bacterial taxa .
	manualset3
255873	2	425877	7	NULL	NULL	NULL	NULL	culture-based methods	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Culture-independent analysis combined with culture-based methods indicated the presence of thermophilic crenarchaeal and gram-positive bacterial taxa .
	manualset3
255874	3	425877	7	NULL	NULL	NULL	NULL	presence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Culture-independent analysis combined with culture-based methods indicated the presence of thermophilic crenarchaeal and gram-positive bacterial taxa .
	manualset3
255875	4	425877	7	NULL	NULL	NULL	NULL	thermophilic crenarchaeal taxa	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Culture-independent analysis combined with culture-based methods indicated the presence of thermophilic crenarchaeal and gram-positive bacterial taxa .
	manualset3
255876	5	425877	7	NULL	NULL	NULL	NULL	gram-positive bacterial taxa	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Culture-independent analysis combined with culture-based methods indicated the presence of thermophilic crenarchaeal and gram-positive bacterial taxa .
	manualset3
255877	1	425878	7	NULL	NULL	NULL	NULL	Culture	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Culture revealed H. pylori in only 69 % of the patients but this pathogen appeared more common when rapid urease tests ( 71 % ) , PCR-denaturating gradient gel electrophoresis ( 91 % ) , histopathology ( 81 % ) , silver staining ( 75 % ) or stool-antigen tests ( 81 % ) were employed .
	manualset3
255878	2	425878	7	NULL	NULL	NULL	NULL	H. pylori	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Culture revealed H. pylori in only 69 % of the patients but this pathogen appeared more common when rapid urease tests ( 71 % ) , PCR-denaturating gradient gel electrophoresis ( 91 % ) , histopathology ( 81 % ) , silver staining ( 75 % ) or stool-antigen tests ( 81 % ) were employed .
	manualset3
255879	3	425878	7	NULL	NULL	NULL	NULL	69 %	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Culture revealed H. pylori in only 69 % of the patients but this pathogen appeared more common when rapid urease tests ( 71 % ) , PCR-denaturating gradient gel electrophoresis ( 91 % ) , histopathology ( 81 % ) , silver staining ( 75 % ) or stool-antigen tests ( 81 % ) were employed .
	manualset3
255880	4	425878	7	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Culture revealed H. pylori in only 69 % of the patients but this pathogen appeared more common when rapid urease tests ( 71 % ) , PCR-denaturating gradient gel electrophoresis ( 91 % ) , histopathology ( 81 % ) , silver staining ( 75 % ) or stool-antigen tests ( 81 % ) were employed .
	manualset3
255881	5	425878	7	NULL	NULL	NULL	NULL	pathogen	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Culture revealed H. pylori in only 69 % of the patients but this pathogen appeared more common when rapid urease tests ( 71 % ) , PCR-denaturating gradient gel electrophoresis ( 91 % ) , histopathology ( 81 % ) , silver staining ( 75 % ) or stool-antigen tests ( 81 % ) were employed .
	manualset3
255882	6	425878	7	NULL	NULL	NULL	NULL	rapid urease tests	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Culture revealed H. pylori in only 69 % of the patients but this pathogen appeared more common when rapid urease tests ( 71 % ) , PCR-denaturating gradient gel electrophoresis ( 91 % ) , histopathology ( 81 % ) , silver staining ( 75 % ) or stool-antigen tests ( 81 % ) were employed .
	manualset3
255883	7	425878	7	NULL	NULL	NULL	NULL	71 %	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Culture revealed H. pylori in only 69 % of the patients but this pathogen appeared more common when rapid urease tests ( 71 % ) , PCR-denaturating gradient gel electrophoresis ( 91 % ) , histopathology ( 81 % ) , silver staining ( 75 % ) or stool-antigen tests ( 81 % ) were employed .
	manualset3
255884	8	425878	7	NULL	NULL	NULL	NULL	PCR-denaturating gradient gel electrophoresis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Culture revealed H. pylori in only 69 % of the patients but this pathogen appeared more common when rapid urease tests ( 71 % ) , PCR-denaturating gradient gel electrophoresis ( 91 % ) , histopathology ( 81 % ) , silver staining ( 75 % ) or stool-antigen tests ( 81 % ) were employed .
	manualset3
255885	9	425878	7	NULL	NULL	NULL	NULL	 91 %	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Culture revealed H. pylori in only 69 % of the patients but this pathogen appeared more common when rapid urease tests ( 71 % ) , PCR-denaturating gradient gel electrophoresis ( 91 % ) , histopathology ( 81 % ) , silver staining ( 75 % ) or stool-antigen tests ( 81 % ) were employed .
	manualset3
255886	10	425878	7	NULL	NULL	NULL	NULL	histopathology	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Culture revealed H. pylori in only 69 % of the patients but this pathogen appeared more common when rapid urease tests ( 71 % ) , PCR-denaturating gradient gel electrophoresis ( 91 % ) , histopathology ( 81 % ) , silver staining ( 75 % ) or stool-antigen tests ( 81 % ) were employed .
	manualset3
255887	11	425878	7	NULL	NULL	NULL	NULL	81 %	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Culture revealed H. pylori in only 69 % of the patients but this pathogen appeared more common when rapid urease tests ( 71 % ) , PCR-denaturating gradient gel electrophoresis ( 91 % ) , histopathology ( 81 % ) , silver staining ( 75 % ) or stool-antigen tests ( 81 % ) were employed .
	manualset3
255888	12	425878	7	NULL	NULL	NULL	NULL	 silver staining 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Culture revealed H. pylori in only 69 % of the patients but this pathogen appeared more common when rapid urease tests ( 71 % ) , PCR-denaturating gradient gel electrophoresis ( 91 % ) , histopathology ( 81 % ) , silver staining ( 75 % ) or stool-antigen tests ( 81 % ) were employed .
	manualset3
255889	13	425878	7	NULL	NULL	NULL	NULL	75 %	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Culture revealed H. pylori in only 69 % of the patients but this pathogen appeared more common when rapid urease tests ( 71 % ) , PCR-denaturating gradient gel electrophoresis ( 91 % ) , histopathology ( 81 % ) , silver staining ( 75 % ) or stool-antigen tests ( 81 % ) were employed .
	manualset3
255890	14	425878	7	NULL	NULL	NULL	NULL	 stool-antigen tests	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Culture revealed H. pylori in only 69 % of the patients but this pathogen appeared more common when rapid urease tests ( 71 % ) , PCR-denaturating gradient gel electrophoresis ( 91 % ) , histopathology ( 81 % ) , silver staining ( 75 % ) or stool-antigen tests ( 81 % ) were employed .
	manualset3
255891	15	425878	7	NULL	NULL	NULL	NULL	81 %	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Culture revealed H. pylori in only 69 % of the patients but this pathogen appeared more common when rapid urease tests ( 71 % ) , PCR-denaturating gradient gel electrophoresis ( 91 % ) , histopathology ( 81 % ) , silver staining ( 75 % ) or stool-antigen tests ( 81 % ) were employed .
	manualset3
255892	1	425879	7	NULL	NULL	NULL	NULL	Cultured rat synovial cells 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultured rat synovial cells generate PGE2 upon stimulation with a factor derived from rate polymorphonuclear cells ( Prostaglandins 27 , 697 , 1984 ) .
	manualset3
255893	2	425879	7	NULL	NULL	NULL	NULL	PGE2	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultured rat synovial cells generate PGE2 upon stimulation with a factor derived from rate polymorphonuclear cells ( Prostaglandins 27 , 697 , 1984 ) .
	manualset3
255894	3	425879	7	NULL	NULL	NULL	NULL	stimulation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultured rat synovial cells generate PGE2 upon stimulation with a factor derived from rate polymorphonuclear cells ( Prostaglandins 27 , 697 , 1984 ) .
	manualset3
255895	4	425879	7	NULL	NULL	NULL	NULL	factor	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultured rat synovial cells generate PGE2 upon stimulation with a factor derived from rate polymorphonuclear cells ( Prostaglandins 27 , 697 , 1984 ) .
	manualset3
255896	6	425879	7	NULL	NULL	NULL	NULL	 Prostaglandins 27 , 697 , 1984	PublicationOrCitation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultured rat synovial cells generate PGE2 upon stimulation with a factor derived from rate polymorphonuclear cells ( Prostaglandins 27 , 697 , 1984 ) .
	manualset3
258943	5	425879	7	NULL	NULL	NULL	NULL	rate polymorphonuclear cells 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultured rat synovial cells generate PGE2 upon stimulation with a factor derived from rate polymorphonuclear cells ( Prostaglandins 27 , 697 , 1984 ) .
	manualset3
255897	1	425880	7	NULL	NULL	NULL	NULL	Cultures	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255898	2	425880	7	NULL	NULL	NULL	NULL	activated endothelial spindle cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255899	3	425880	7	NULL	NULL	NULL	NULL	hyperplastic 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255900	4	425880	7	NULL	NULL	NULL	NULL	neoplastic	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255901	5	425880	7	NULL	NULL	NULL	NULL	HHV-8	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255902	6	425880	7	NULL	NULL	NULL	NULL	transmission	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255903	7	425880	7	NULL	NULL	NULL	NULL	HHV-8	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255904	8	425880	7	NULL	NULL	NULL	NULL	cell growth	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255905	9	425880	7	NULL	NULL	NULL	NULL	transformation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255906	10	425880	7	NULL	NULL	NULL	NULL	monkeys immune	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255907	11	425880	7	NULL	NULL	NULL	NULL	simian immunodeficiency virus infection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255908	12	425880	7	NULL	NULL	NULL	NULL	HHV-8	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255909	13	425880	7	NULL	NULL	NULL	NULL	KS	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255910	14	425880	7	NULL	NULL	NULL	NULL	polymerase chain reaction analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255911	15	425880	7	NULL	NULL	NULL	NULL	blood cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255912	16	425880	7	NULL	NULL	NULL	NULL	HHV-8 sequences	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255913	17	425880	7	NULL	NULL	NULL	NULL	monocytes	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255914	18	425880	7	NULL	NULL	NULL	NULL	B cells 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255915	19	425880	7	NULL	NULL	NULL	NULL	20 % 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255916	20	425880	7	NULL	NULL	NULL	NULL	normal donors	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255917	21	425880	7	NULL	NULL	NULL	NULL	Maryland	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255918	22	425880	7	NULL	NULL	NULL	NULL	M. Starzl 	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255919	23	425880	7	NULL	NULL	NULL	NULL	early KS	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255920	24	425880	7	NULL	NULL	NULL	NULL	cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255921	25	425880	7	NULL	NULL	NULL	NULL	 macrophage	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255922	26	425880	7	NULL	NULL	NULL	NULL	HHV-8	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255923	27	425880	7	NULL	NULL	NULL	NULL	endothelial cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255924	28	425880	7	NULL	NULL	NULL	NULL	late 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255925	29	425880	7	NULL	NULL	NULL	NULL	 disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255926	30	425880	7	NULL	NULL	NULL	NULL	increase	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255927	31	425880	7	NULL	NULL	NULL	NULL	HHV-8	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255928	32	425880	7	NULL	NULL	NULL	NULL	association	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255929	33	425880	7	NULL	NULL	NULL	NULL	progressive immune deficiency	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255930	34	425880	7	NULL	NULL	NULL	NULL	recent studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255931	35	425880	7	NULL	NULL	NULL	NULL	 Gambia	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255932	36	425880	7	NULL	NULL	NULL	NULL	 HHV-8	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255933	37	425880	7	NULL	NULL	NULL	NULL	common infection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255934	38	425880	7	NULL	NULL	NULL	NULL	HHV-2	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255935	39	425880	7	NULL	NULL	NULL	NULL	HIV-1	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255936	40	425880	7	NULL	NULL	NULL	NULL	 KS	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of all activated endothelial spindle cells , whether hyperplastic or neoplastic , are negative for HHV-8 ; transmission of HHV-8 does not induce cell growth or transformation ; monkeys immune suppressed by simian immunodeficiency virus infection and infected also with HHV-8 do not develop KS ; polymerase chain reaction analysis of blood cells shows HHV-8 sequences in monocytes and B cells ( about 20 % of normal donors in Maryland ) ; M. Starzl showed that early KS has few cells ( mostly macrophage ) positive for HHV-8 , increasing and present in endothelial cells only late in the disease ; no increase in HHV-8 has been found in association with progressive immune deficiency ; and recent studies in Gambia by others showed that HHV-8 is a very common infection , and though HHV-2 is known to be relatively common , HIV-1 is unusual and so is KS .
	manualset3
255937	1	425881	7	NULL	NULL	NULL	NULL	Cultures	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of human peripheral blood lymphocytes were maintained for 21 days in the presence of subthreshold concentration of PHA .
	manualset3
255938	2	425881	7	NULL	NULL	NULL	NULL	 human peripheral blood lymphocytes	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of human peripheral blood lymphocytes were maintained for 21 days in the presence of subthreshold concentration of PHA .
	manualset3
255939	3	425881	7	NULL	NULL	NULL	NULL	21 days	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of human peripheral blood lymphocytes were maintained for 21 days in the presence of subthreshold concentration of PHA .
	manualset3
255940	4	425881	7	NULL	NULL	NULL	NULL	presence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of human peripheral blood lymphocytes were maintained for 21 days in the presence of subthreshold concentration of PHA .
	manualset3
255941	5	425881	7	NULL	NULL	NULL	NULL	subthreshold concentration	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of human peripheral blood lymphocytes were maintained for 21 days in the presence of subthreshold concentration of PHA .
	manualset3
255942	6	425881	7	NULL	NULL	NULL	NULL	PHA	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures of human peripheral blood lymphocytes were maintained for 21 days in the presence of subthreshold concentration of PHA .
	manualset3
255943	1	425882	7	NULL	NULL	NULL	NULL	Cultures	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures using natural leaf litter from beneath beech trees had higher densities and diversity of gymnamoebae than leaf-litter cultures from a maple-oak stand .
	manualset3
255944	2	425882	7	NULL	NULL	NULL	NULL	natural leaf litter	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures using natural leaf litter from beneath beech trees had higher densities and diversity of gymnamoebae than leaf-litter cultures from a maple-oak stand .
	manualset3
255945	3	425882	7	NULL	NULL	NULL	NULL	beneath beech trees	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures using natural leaf litter from beneath beech trees had higher densities and diversity of gymnamoebae than leaf-litter cultures from a maple-oak stand .
	manualset3
255946	4	425882	7	NULL	NULL	NULL	NULL	higher densities	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures using natural leaf litter from beneath beech trees had higher densities and diversity of gymnamoebae than leaf-litter cultures from a maple-oak stand .
	manualset3
255947	5	425882	7	NULL	NULL	NULL	NULL	diversity	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures using natural leaf litter from beneath beech trees had higher densities and diversity of gymnamoebae than leaf-litter cultures from a maple-oak stand .
	manualset3
255948	6	425882	7	NULL	NULL	NULL	NULL	gymnamoebae	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures using natural leaf litter from beneath beech trees had higher densities and diversity of gymnamoebae than leaf-litter cultures from a maple-oak stand .
	manualset3
255949	7	425882	7	NULL	NULL	NULL	NULL	leaf-litter cultures	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures using natural leaf litter from beneath beech trees had higher densities and diversity of gymnamoebae than leaf-litter cultures from a maple-oak stand .
	manualset3
255950	8	425882	7	NULL	NULL	NULL	NULL	maple-oak stand	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cultures using natural leaf litter from beneath beech trees had higher densities and diversity of gymnamoebae than leaf-litter cultures from a maple-oak stand .
	manualset3
255951	1	425883	7	NULL	NULL	NULL	NULL	Cumulative Na balance	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulative Na balance was greater in CBDL and CHF rats , INN or DNX , than in Sham/CBDL or CHF rats throughout the study .
	manualset3
255952	2	425883	7	NULL	NULL	NULL	NULL	CBDL rats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulative Na balance was greater in CBDL and CHF rats , INN or DNX , than in Sham/CBDL or CHF rats throughout the study .
	manualset3
255953	3	425883	7	NULL	NULL	NULL	NULL	CHF rats 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulative Na balance was greater in CBDL and CHF rats , INN or DNX , than in Sham/CBDL or CHF rats throughout the study .
	manualset3
255954	4	425883	7	NULL	NULL	NULL	NULL	INN	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulative Na balance was greater in CBDL and CHF rats , INN or DNX , than in Sham/CBDL or CHF rats throughout the study .
	manualset3
255955	5	425883	7	NULL	NULL	NULL	NULL	DNX	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulative Na balance was greater in CBDL and CHF rats , INN or DNX , than in Sham/CBDL or CHF rats throughout the study .
	manualset3
255956	6	425883	7	NULL	NULL	NULL	NULL	Sham/CBDL rats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulative Na balance was greater in CBDL and CHF rats , INN or DNX , than in Sham/CBDL or CHF rats throughout the study .
	manualset3
255957	7	425883	7	NULL	NULL	NULL	NULL	CHF rats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulative Na balance was greater in CBDL and CHF rats , INN or DNX , than in Sham/CBDL or CHF rats throughout the study .
	manualset3
255958	8	425883	7	NULL	NULL	NULL	NULL	study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulative Na balance was greater in CBDL and CHF rats , INN or DNX , than in Sham/CBDL or CHF rats throughout the study .
	manualset3
255959	1	425884	7	NULL	NULL	NULL	NULL	Cumulative title list	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulative title list of dissertations in the field of surgery and related specialities .
	manualset3
255960	2	425884	7	NULL	NULL	NULL	NULL	dissertations	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulative title list of dissertations in the field of surgery and related specialities .
	manualset3
255961	3	425884	7	NULL	NULL	NULL	NULL	 field	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulative title list of dissertations in the field of surgery and related specialities .
	manualset3
255962	5	425884	7	NULL	NULL	NULL	NULL	specialities	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulative title list of dissertations in the field of surgery and related specialities .
	manualset3
258959	4	425884	7	NULL	NULL	NULL	NULL	surgery	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulative title list of dissertations in the field of surgery and related specialities .
	manualset3
255963	1	425885	7	NULL	NULL	NULL	NULL	Medical prescription	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Medical prescription of psychiatric drugs in primary care ) .
	manualset3
255964	2	425885	7	NULL	NULL	NULL	NULL	psychiatric drugs	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Medical prescription of psychiatric drugs in primary care ) .
	manualset3
255965	3	425885	7	NULL	NULL	NULL	NULL	primary care 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Medical prescription of psychiatric drugs in primary care ) .
	manualset3
256058	1	425886	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulatively , these results suggest that TLR2 signaling enhances Nox1 expression through the JAK1/3-STAT 3 pathway , and that RGS2 , through its regulation by the PKC - / PLD2 pathway , represses STAT3 's transcriptional activation of Nox1 .
	manualset3
256059	2	425886	7	NULL	NULL	NULL	NULL	TLR2 signaling	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulatively , these results suggest that TLR2 signaling enhances Nox1 expression through the JAK1/3-STAT 3 pathway , and that RGS2 , through its regulation by the PKC - / PLD2 pathway , represses STAT3 's transcriptional activation of Nox1 .
	manualset3
256060	3	425886	7	NULL	NULL	NULL	NULL	Nox1 expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulatively , these results suggest that TLR2 signaling enhances Nox1 expression through the JAK1/3-STAT 3 pathway , and that RGS2 , through its regulation by the PKC - / PLD2 pathway , represses STAT3 's transcriptional activation of Nox1 .
	manualset3
256061	4	425886	7	NULL	NULL	NULL	NULL	JAK1/3-STAT 3 pathway	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulatively , these results suggest that TLR2 signaling enhances Nox1 expression through the JAK1/3-STAT 3 pathway , and that RGS2 , through its regulation by the PKC - / PLD2 pathway , represses STAT3 's transcriptional activation of Nox1 .
	manualset3
256062	5	425886	7	NULL	NULL	NULL	NULL	RGS2	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulatively , these results suggest that TLR2 signaling enhances Nox1 expression through the JAK1/3-STAT 3 pathway , and that RGS2 , through its regulation by the PKC - / PLD2 pathway , represses STAT3 's transcriptional activation of Nox1 .
	manualset3
256063	6	425886	7	NULL	NULL	NULL	NULL	regulation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulatively , these results suggest that TLR2 signaling enhances Nox1 expression through the JAK1/3-STAT 3 pathway , and that RGS2 , through its regulation by the PKC - / PLD2 pathway , represses STAT3 's transcriptional activation of Nox1 .
	manualset3
256064	7	425886	7	NULL	NULL	NULL	NULL	PKC - / PLD2 pathway	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulatively , these results suggest that TLR2 signaling enhances Nox1 expression through the JAK1/3-STAT 3 pathway , and that RGS2 , through its regulation by the PKC - / PLD2 pathway , represses STAT3 's transcriptional activation of Nox1 .
	manualset3
256065	8	425886	7	NULL	NULL	NULL	NULL	STAT3 's transcriptional activation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulatively , these results suggest that TLR2 signaling enhances Nox1 expression through the JAK1/3-STAT 3 pathway , and that RGS2 , through its regulation by the PKC - / PLD2 pathway , represses STAT3 's transcriptional activation of Nox1 .
	manualset3
256066	9	425886	7	NULL	NULL	NULL	NULL	Nox1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulatively , these results suggest that TLR2 signaling enhances Nox1 expression through the JAK1/3-STAT 3 pathway , and that RGS2 , through its regulation by the PKC - / PLD2 pathway , represses STAT3 's transcriptional activation of Nox1 .
	manualset3
256067	1	425887	7	NULL	NULL	NULL	NULL	Cumulus cell-enclosed oocytes	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulus cell-enclosed oocytes that were compromised in their ability to undergo nuclear maturation and subsequent development because of the age or genotype of the female were isolated at the germinal vesicle stage and matured in vitro using media supplemented with 0 to 20 microM FF-MAS .
	manualset3
256068	2	425887	7	NULL	NULL	NULL	NULL	ability	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulus cell-enclosed oocytes that were compromised in their ability to undergo nuclear maturation and subsequent development because of the age or genotype of the female were isolated at the germinal vesicle stage and matured in vitro using media supplemented with 0 to 20 microM FF-MAS .
	manualset3
256069	3	425887	7	NULL	NULL	NULL	NULL	nuclear maturation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulus cell-enclosed oocytes that were compromised in their ability to undergo nuclear maturation and subsequent development because of the age or genotype of the female were isolated at the germinal vesicle stage and matured in vitro using media supplemented with 0 to 20 microM FF-MAS .
	manualset3
256070	4	425887	7	NULL	NULL	NULL	NULL	development 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulus cell-enclosed oocytes that were compromised in their ability to undergo nuclear maturation and subsequent development because of the age or genotype of the female were isolated at the germinal vesicle stage and matured in vitro using media supplemented with 0 to 20 microM FF-MAS .
	manualset3
256071	5	425887	7	NULL	NULL	NULL	NULL	age	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulus cell-enclosed oocytes that were compromised in their ability to undergo nuclear maturation and subsequent development because of the age or genotype of the female were isolated at the germinal vesicle stage and matured in vitro using media supplemented with 0 to 20 microM FF-MAS .
	manualset3
256072	6	425887	7	NULL	NULL	NULL	NULL	genotype	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulus cell-enclosed oocytes that were compromised in their ability to undergo nuclear maturation and subsequent development because of the age or genotype of the female were isolated at the germinal vesicle stage and matured in vitro using media supplemented with 0 to 20 microM FF-MAS .
	manualset3
256073	7	425887	7	NULL	NULL	NULL	NULL	 female	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulus cell-enclosed oocytes that were compromised in their ability to undergo nuclear maturation and subsequent development because of the age or genotype of the female were isolated at the germinal vesicle stage and matured in vitro using media supplemented with 0 to 20 microM FF-MAS .
	manualset3
256074	8	425887	7	NULL	NULL	NULL	NULL	germinal vesicle stage	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulus cell-enclosed oocytes that were compromised in their ability to undergo nuclear maturation and subsequent development because of the age or genotype of the female were isolated at the germinal vesicle stage and matured in vitro using media supplemented with 0 to 20 microM FF-MAS .
	manualset3
256075	9	425887	7	NULL	NULL	NULL	NULL	0 to 20 microM	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulus cell-enclosed oocytes that were compromised in their ability to undergo nuclear maturation and subsequent development because of the age or genotype of the female were isolated at the germinal vesicle stage and matured in vitro using media supplemented with 0 to 20 microM FF-MAS .
	manualset3
256076	10	425887	7	NULL	NULL	NULL	NULL	FF-MAS	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulus cell-enclosed oocytes that were compromised in their ability to undergo nuclear maturation and subsequent development because of the age or genotype of the female were isolated at the germinal vesicle stage and matured in vitro using media supplemented with 0 to 20 microM FF-MAS .
	manualset3
258960	11	425887	7	NULL	NULL	NULL	NULL	media	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cumulus cell-enclosed oocytes that were compromised in their ability to undergo nuclear maturation and subsequent development because of the age or genotype of the female were isolated at the germinal vesicle stage and matured in vitro using media supplemented with 0 to 20 microM FF-MAS .
	manualset3
256077	1	425888	7	NULL	NULL	NULL	NULL	Curative resection	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Curative resection was performed upon ten of 26 patients who underwent operation .
	manualset3
256078	2	425888	7	NULL	NULL	NULL	NULL	ten	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Curative resection was performed upon ten of 26 patients who underwent operation .
	manualset3
256079	3	425888	7	NULL	NULL	NULL	NULL	26 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Curative resection was performed upon ten of 26 patients who underwent operation .
	manualset3
256080	4	425888	7	NULL	NULL	NULL	NULL	operation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Curative resection was performed upon ten of 26 patients who underwent operation .
	manualset3
256081	1	425889	7	NULL	NULL	NULL	NULL	Curcumin	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Curcumin mediated apoptosis in these cells appears to be due to upregulation of proapoptotic Bax , AIF , release of cytochrome c and down regulation of antiapoptotic Bcl-2 , Bcl-XL in HeLa and SiHa .
	manualset3
256082	2	425889	7	NULL	NULL	NULL	NULL	apoptosis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Curcumin mediated apoptosis in these cells appears to be due to upregulation of proapoptotic Bax , AIF , release of cytochrome c and down regulation of antiapoptotic Bcl-2 , Bcl-XL in HeLa and SiHa .
	manualset3
256083	3	425889	7	NULL	NULL	NULL	NULL	cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Curcumin mediated apoptosis in these cells appears to be due to upregulation of proapoptotic Bax , AIF , release of cytochrome c and down regulation of antiapoptotic Bcl-2 , Bcl-XL in HeLa and SiHa .
	manualset3
256084	4	425889	7	NULL	NULL	NULL	NULL	upregulation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Curcumin mediated apoptosis in these cells appears to be due to upregulation of proapoptotic Bax , AIF , release of cytochrome c and down regulation of antiapoptotic Bcl-2 , Bcl-XL in HeLa and SiHa .
	manualset3
256085	5	425889	7	NULL	NULL	NULL	NULL	proapoptotic Bax 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Curcumin mediated apoptosis in these cells appears to be due to upregulation of proapoptotic Bax , AIF , release of cytochrome c and down regulation of antiapoptotic Bcl-2 , Bcl-XL in HeLa and SiHa .
	manualset3
256086	6	425889	7	NULL	NULL	NULL	NULL	AIF	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Curcumin mediated apoptosis in these cells appears to be due to upregulation of proapoptotic Bax , AIF , release of cytochrome c and down regulation of antiapoptotic Bcl-2 , Bcl-XL in HeLa and SiHa .
	manualset3
256087	7	425889	7	NULL	NULL	NULL	NULL	release	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Curcumin mediated apoptosis in these cells appears to be due to upregulation of proapoptotic Bax , AIF , release of cytochrome c and down regulation of antiapoptotic Bcl-2 , Bcl-XL in HeLa and SiHa .
	manualset3
256088	8	425889	7	NULL	NULL	NULL	NULL	cytochrome c	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Curcumin mediated apoptosis in these cells appears to be due to upregulation of proapoptotic Bax , AIF , release of cytochrome c and down regulation of antiapoptotic Bcl-2 , Bcl-XL in HeLa and SiHa .
	manualset3
256089	9	425889	7	NULL	NULL	NULL	NULL	down regulation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Curcumin mediated apoptosis in these cells appears to be due to upregulation of proapoptotic Bax , AIF , release of cytochrome c and down regulation of antiapoptotic Bcl-2 , Bcl-XL in HeLa and SiHa .
	manualset3
256090	10	425889	7	NULL	NULL	NULL	NULL	antiapoptotic Bcl-2	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Curcumin mediated apoptosis in these cells appears to be due to upregulation of proapoptotic Bax , AIF , release of cytochrome c and down regulation of antiapoptotic Bcl-2 , Bcl-XL in HeLa and SiHa .
	manualset3
256091	11	425889	7	NULL	NULL	NULL	NULL	Bcl-XL	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Curcumin mediated apoptosis in these cells appears to be due to upregulation of proapoptotic Bax , AIF , release of cytochrome c and down regulation of antiapoptotic Bcl-2 , Bcl-XL in HeLa and SiHa .
	manualset3
256092	12	425889	7	NULL	NULL	NULL	NULL	HeLa 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Curcumin mediated apoptosis in these cells appears to be due to upregulation of proapoptotic Bax , AIF , release of cytochrome c and down regulation of antiapoptotic Bcl-2 , Bcl-XL in HeLa and SiHa .
	manualset3
256093	13	425889	7	NULL	NULL	NULL	NULL	SiHa	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Curcumin mediated apoptosis in these cells appears to be due to upregulation of proapoptotic Bax , AIF , release of cytochrome c and down regulation of antiapoptotic Bcl-2 , Bcl-XL in HeLa and SiHa .
	manualset3
256094	1	425890	7	NULL	NULL	NULL	NULL	Cured animals	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cured animals rejected a challenge of E7-expressing tumors , such as TC-1 and B16E7 , but not a challenge of B16 7 weeks after the combined treatment , showing antigen-specific immune responses .
	manualset3
256095	2	425890	7	NULL	NULL	NULL	NULL	 challenge	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cured animals rejected a challenge of E7-expressing tumors , such as TC-1 and B16E7 , but not a challenge of B16 7 weeks after the combined treatment , showing antigen-specific immune responses .
	manualset3
256096	3	425890	7	NULL	NULL	NULL	NULL	 E7-expressing tumors	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cured animals rejected a challenge of E7-expressing tumors , such as TC-1 and B16E7 , but not a challenge of B16 7 weeks after the combined treatment , showing antigen-specific immune responses .
	manualset3
256097	4	425890	7	NULL	NULL	NULL	NULL	 TC-1	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cured animals rejected a challenge of E7-expressing tumors , such as TC-1 and B16E7 , but not a challenge of B16 7 weeks after the combined treatment , showing antigen-specific immune responses .
	manualset3
256098	5	425890	7	NULL	NULL	NULL	NULL	B16E7	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cured animals rejected a challenge of E7-expressing tumors , such as TC-1 and B16E7 , but not a challenge of B16 7 weeks after the combined treatment , showing antigen-specific immune responses .
	manualset3
256099	6	425890	7	NULL	NULL	NULL	NULL	B16	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cured animals rejected a challenge of E7-expressing tumors , such as TC-1 and B16E7 , but not a challenge of B16 7 weeks after the combined treatment , showing antigen-specific immune responses .
	manualset3
256100	7	425890	7	NULL	NULL	NULL	NULL	7 weeks	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cured animals rejected a challenge of E7-expressing tumors , such as TC-1 and B16E7 , but not a challenge of B16 7 weeks after the combined treatment , showing antigen-specific immune responses .
	manualset3
256101	8	425890	7	NULL	NULL	NULL	NULL	combined treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cured animals rejected a challenge of E7-expressing tumors , such as TC-1 and B16E7 , but not a challenge of B16 7 weeks after the combined treatment , showing antigen-specific immune responses .
	manualset3
256102	9	425890	7	NULL	NULL	NULL	NULL	antigen-specific immune responses	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cured animals rejected a challenge of E7-expressing tumors , such as TC-1 and B16E7 , but not a challenge of B16 7 weeks after the combined treatment , showing antigen-specific immune responses .
	manualset3
256103	1	425891	7	NULL	NULL	NULL	NULL	Curing time	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Curing time was kept as low as possible to improve entrapment with increasing drug concentration .
	manualset3
256104	2	425891	7	NULL	NULL	NULL	NULL	entrapment 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Curing time was kept as low as possible to improve entrapment with increasing drug concentration .
	manualset3
256105	3	425891	7	NULL	NULL	NULL	NULL	drug concentration	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Curing time was kept as low as possible to improve entrapment with increasing drug concentration .
	manualset3
256106	1	425892	7	NULL	NULL	NULL	NULL	olfactory system	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Curiously , the olfactory system is rather immature at birth and undergoes a maturation process , which is poorly understood .
	manualset3
256107	2	425892	7	NULL	NULL	NULL	NULL	 birth	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Curiously , the olfactory system is rather immature at birth and undergoes a maturation process , which is poorly understood .
	manualset3
256108	3	425892	7	NULL	NULL	NULL	NULL	maturation process	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Curiously , the olfactory system is rather immature at birth and undergoes a maturation process , which is poorly understood .
	manualset3
256109	1	425893	7	NULL	NULL	NULL	NULL	Current animal models 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current animal models of bronchial asthma .
	manualset3
256110	2	425893	7	NULL	NULL	NULL	NULL	bronchial asthma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current animal models of bronchial asthma .
	manualset3
256111	1	425894	7	NULL	NULL	NULL	NULL	Medicine 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Medicine and music in the head .
	manualset3
256112	2	425894	7	NULL	NULL	NULL	NULL	music	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Medicine and music in the head .
	manualset3
256113	3	425894	7	NULL	NULL	NULL	NULL	head	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Medicine and music in the head .
	manualset3
256114	1	425895	7	NULL	NULL	NULL	NULL	Current concepts	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current concepts in nutrition : enteral tube feeding .
	manualset3
256115	2	425895	7	NULL	NULL	NULL	NULL	nutrition	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current concepts in nutrition : enteral tube feeding .
	manualset3
256116	3	425895	7	NULL	NULL	NULL	NULL	enteral tube feeding 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current concepts in nutrition : enteral tube feeding .
	manualset3
256117	1	425896	7	NULL	NULL	NULL	NULL	Current concepts review	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current concepts review : septic arthritis of the knee pathophysiology , diagnostics , and therapy .
	manualset3
256118	2	425896	7	NULL	NULL	NULL	NULL	septic arthritis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current concepts review : septic arthritis of the knee pathophysiology , diagnostics , and therapy .
	manualset3
256119	3	425896	7	NULL	NULL	NULL	NULL	 knee pathophysiology	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current concepts review : septic arthritis of the knee pathophysiology , diagnostics , and therapy .
	manualset3
256120	4	425896	7	NULL	NULL	NULL	NULL	diagnostics	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current concepts review : septic arthritis of the knee pathophysiology , diagnostics , and therapy .
	manualset3
256121	5	425896	7	NULL	NULL	NULL	NULL	therapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current concepts review : septic arthritis of the knee pathophysiology , diagnostics , and therapy .
	manualset3
256122	1	425897	7	NULL	NULL	NULL	NULL	Current diagnostic protocols	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current diagnostic protocols depend substantially on cytology as an initial diagnostic modality .
	manualset3
256123	2	425897	7	NULL	NULL	NULL	NULL	cytology	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current diagnostic protocols depend substantially on cytology as an initial diagnostic modality .
	manualset3
256124	3	425897	7	NULL	NULL	NULL	NULL	initial diagnostic modality	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current diagnostic protocols depend substantially on cytology as an initial diagnostic modality .
	manualset3
256125	1	425898	7	NULL	NULL	NULL	NULL	Current guidelines	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current guidelines for the radiological assessment of MM still recommend the traditional skeletal survey , although its limitations are well documented , especially in early phases of the disease when radiographs can significantly underestimate the extent of bone lesions and bone marrow involvement .
	manualset3
256126	2	425898	7	NULL	NULL	NULL	NULL	radiological assessment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current guidelines for the radiological assessment of MM still recommend the traditional skeletal survey , although its limitations are well documented , especially in early phases of the disease when radiographs can significantly underestimate the extent of bone lesions and bone marrow involvement .
	manualset3
256127	3	425898	7	NULL	NULL	NULL	NULL	MM	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current guidelines for the radiological assessment of MM still recommend the traditional skeletal survey , although its limitations are well documented , especially in early phases of the disease when radiographs can significantly underestimate the extent of bone lesions and bone marrow involvement .
	manualset3
256128	4	425898	7	NULL	NULL	NULL	NULL	 traditional skeletal survey	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current guidelines for the radiological assessment of MM still recommend the traditional skeletal survey , although its limitations are well documented , especially in early phases of the disease when radiographs can significantly underestimate the extent of bone lesions and bone marrow involvement .
	manualset3
256129	5	425898	7	NULL	NULL	NULL	NULL	limitations	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current guidelines for the radiological assessment of MM still recommend the traditional skeletal survey , although its limitations are well documented , especially in early phases of the disease when radiographs can significantly underestimate the extent of bone lesions and bone marrow involvement .
	manualset3
256130	6	425898	7	NULL	NULL	NULL	NULL	early phases	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current guidelines for the radiological assessment of MM still recommend the traditional skeletal survey , although its limitations are well documented , especially in early phases of the disease when radiographs can significantly underestimate the extent of bone lesions and bone marrow involvement .
	manualset3
256131	7	425898	7	NULL	NULL	NULL	NULL	disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current guidelines for the radiological assessment of MM still recommend the traditional skeletal survey , although its limitations are well documented , especially in early phases of the disease when radiographs can significantly underestimate the extent of bone lesions and bone marrow involvement .
	manualset3
256132	8	425898	7	NULL	NULL	NULL	NULL	radiographs	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current guidelines for the radiological assessment of MM still recommend the traditional skeletal survey , although its limitations are well documented , especially in early phases of the disease when radiographs can significantly underestimate the extent of bone lesions and bone marrow involvement .
	manualset3
256133	9	425898	7	NULL	NULL	NULL	NULL	extent 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current guidelines for the radiological assessment of MM still recommend the traditional skeletal survey , although its limitations are well documented , especially in early phases of the disease when radiographs can significantly underestimate the extent of bone lesions and bone marrow involvement .
	manualset3
256134	10	425898	7	NULL	NULL	NULL	NULL	 bone lesions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current guidelines for the radiological assessment of MM still recommend the traditional skeletal survey , although its limitations are well documented , especially in early phases of the disease when radiographs can significantly underestimate the extent of bone lesions and bone marrow involvement .
	manualset3
256135	11	425898	7	NULL	NULL	NULL	NULL	 bone marrow involvement	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current guidelines for the radiological assessment of MM still recommend the traditional skeletal survey , although its limitations are well documented , especially in early phases of the disease when radiographs can significantly underestimate the extent of bone lesions and bone marrow involvement .
	manualset3
256136	1	425899	7	NULL	NULL	NULL	NULL	Current knowledge 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current knowledge concerning photosensitivity in SLOS is reviewed and future research into the pathogenesis of this disorder is discussed .
	manualset3
256137	2	425899	7	NULL	NULL	NULL	NULL	photosensitivity	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current knowledge concerning photosensitivity in SLOS is reviewed and future research into the pathogenesis of this disorder is discussed .
	manualset3
256138	3	425899	7	NULL	NULL	NULL	NULL	SLOS	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current knowledge concerning photosensitivity in SLOS is reviewed and future research into the pathogenesis of this disorder is discussed .
	manualset3
256139	4	425899	7	NULL	NULL	NULL	NULL	future research	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current knowledge concerning photosensitivity in SLOS is reviewed and future research into the pathogenesis of this disorder is discussed .
	manualset3
256140	5	425899	7	NULL	NULL	NULL	NULL	pathogenesis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current knowledge concerning photosensitivity in SLOS is reviewed and future research into the pathogenesis of this disorder is discussed .
	manualset3
256141	6	425899	7	NULL	NULL	NULL	NULL	disorder	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current knowledge concerning photosensitivity in SLOS is reviewed and future research into the pathogenesis of this disorder is discussed .
	manualset3
256142	1	425900	7	NULL	NULL	NULL	NULL	Current knowledge gaps	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current knowledge gaps should be fully disclosed to parents , and hydroxyurea therapy should be reserved for patients with severe pain .
	manualset3
256143	2	425900	7	NULL	NULL	NULL	NULL	parents 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current knowledge gaps should be fully disclosed to parents , and hydroxyurea therapy should be reserved for patients with severe pain .
	manualset3
256144	3	425900	7	NULL	NULL	NULL	NULL	hydroxyurea therapy 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current knowledge gaps should be fully disclosed to parents , and hydroxyurea therapy should be reserved for patients with severe pain .
	manualset3
256145	4	425900	7	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current knowledge gaps should be fully disclosed to parents , and hydroxyurea therapy should be reserved for patients with severe pain .
	manualset3
256146	5	425900	7	NULL	NULL	NULL	NULL	severe pain	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current knowledge gaps should be fully disclosed to parents , and hydroxyurea therapy should be reserved for patients with severe pain .
	manualset3
256147	1	425901	7	NULL	NULL	NULL	NULL	metabonomic practice	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current metabonomic practice has relied on mass spectrometry ( MS ) , gas chromatography-mass spectrometry ( GC-MS ) , and nuclear magnetic resonance ( NMR ) to analyze metabolites .
	manualset3
256148	2	425901	7	NULL	NULL	NULL	NULL	mass spectrometry ( MS )	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current metabonomic practice has relied on mass spectrometry ( MS ) , gas chromatography-mass spectrometry ( GC-MS ) , and nuclear magnetic resonance ( NMR ) to analyze metabolites .
	manualset3
256149	3	425901	7	NULL	NULL	NULL	NULL	gas chromatography-mass spectrometry ( GC-MS )	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current metabonomic practice has relied on mass spectrometry ( MS ) , gas chromatography-mass spectrometry ( GC-MS ) , and nuclear magnetic resonance ( NMR ) to analyze metabolites .
	manualset3
256150	4	425901	7	NULL	NULL	NULL	NULL	nuclear magnetic resonance ( NMR )	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current metabonomic practice has relied on mass spectrometry ( MS ) , gas chromatography-mass spectrometry ( GC-MS ) , and nuclear magnetic resonance ( NMR ) to analyze metabolites .
	manualset3
256151	5	425901	7	NULL	NULL	NULL	NULL	metabolites 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current metabonomic practice has relied on mass spectrometry ( MS ) , gas chromatography-mass spectrometry ( GC-MS ) , and nuclear magnetic resonance ( NMR ) to analyze metabolites .
	manualset3
256152	1	425902	7	NULL	NULL	NULL	NULL	Current models	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current models for determining first-order rate coefficients ( k ) from PPTs assume complete and instantaneous mixing of injected test solution in the portion of the aquifer investigated by the test , i.e. , the system is treated like a well-mixed reactor .
	manualset3
256153	2	425902	7	NULL	NULL	NULL	NULL	first-order rate coefficients ( k )	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current models for determining first-order rate coefficients ( k ) from PPTs assume complete and instantaneous mixing of injected test solution in the portion of the aquifer investigated by the test , i.e. , the system is treated like a well-mixed reactor .
	manualset3
256154	3	425902	7	NULL	NULL	NULL	NULL	 PPTs	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current models for determining first-order rate coefficients ( k ) from PPTs assume complete and instantaneous mixing of injected test solution in the portion of the aquifer investigated by the test , i.e. , the system is treated like a well-mixed reactor .
	manualset3
256155	4	425902	7	NULL	NULL	NULL	NULL	 instantaneous mixing	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current models for determining first-order rate coefficients ( k ) from PPTs assume complete and instantaneous mixing of injected test solution in the portion of the aquifer investigated by the test , i.e. , the system is treated like a well-mixed reactor .
	manualset3
256156	5	425902	7	NULL	NULL	NULL	NULL	 injected test solution	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current models for determining first-order rate coefficients ( k ) from PPTs assume complete and instantaneous mixing of injected test solution in the portion of the aquifer investigated by the test , i.e. , the system is treated like a well-mixed reactor .
	manualset3
256157	6	425902	7	NULL	NULL	NULL	NULL	portion 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current models for determining first-order rate coefficients ( k ) from PPTs assume complete and instantaneous mixing of injected test solution in the portion of the aquifer investigated by the test , i.e. , the system is treated like a well-mixed reactor .
	manualset3
256158	7	425902	7	NULL	NULL	NULL	NULL	aquifer	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current models for determining first-order rate coefficients ( k ) from PPTs assume complete and instantaneous mixing of injected test solution in the portion of the aquifer investigated by the test , i.e. , the system is treated like a well-mixed reactor .
	manualset3
256159	8	425902	7	NULL	NULL	NULL	NULL	test 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current models for determining first-order rate coefficients ( k ) from PPTs assume complete and instantaneous mixing of injected test solution in the portion of the aquifer investigated by the test , i.e. , the system is treated like a well-mixed reactor .
	manualset3
256160	9	425902	7	NULL	NULL	NULL	NULL	system 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current models for determining first-order rate coefficients ( k ) from PPTs assume complete and instantaneous mixing of injected test solution in the portion of the aquifer investigated by the test , i.e. , the system is treated like a well-mixed reactor .
	manualset3
256161	10	425902	7	NULL	NULL	NULL	NULL	well-mixed reactor	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current models for determining first-order rate coefficients ( k ) from PPTs assume complete and instantaneous mixing of injected test solution in the portion of the aquifer investigated by the test , i.e. , the system is treated like a well-mixed reactor .
	manualset3
256162	1	425903	7	NULL	NULL	NULL	NULL	Medico-legal considerations	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Medico-legal considerations on a case of food poisoning due to enterotoxic staphylococci ) .
	manualset3
256163	2	425903	7	NULL	NULL	NULL	NULL	case 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Medico-legal considerations on a case of food poisoning due to enterotoxic staphylococci ) .
	manualset3
256164	3	425903	7	NULL	NULL	NULL	NULL	food poisoning	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Medico-legal considerations on a case of food poisoning due to enterotoxic staphylococci ) .
	manualset3
256165	4	425903	7	NULL	NULL	NULL	NULL	enterotoxic staphylococci	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Medico-legal considerations on a case of food poisoning due to enterotoxic staphylococci ) .
	manualset3
256166	1	425904	7	NULL	NULL	NULL	NULL	Current research	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current research is focused on the role of adipokines such as adiponectin and immune cells , especially macrophages , in adipose tissue .
	manualset3
256167	2	425904	7	NULL	NULL	NULL	NULL	role	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current research is focused on the role of adipokines such as adiponectin and immune cells , especially macrophages , in adipose tissue .
	manualset3
256168	3	425904	7	NULL	NULL	NULL	NULL	adipokines	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current research is focused on the role of adipokines such as adiponectin and immune cells , especially macrophages , in adipose tissue .
	manualset3
256169	4	425904	7	NULL	NULL	NULL	NULL	adiponectin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current research is focused on the role of adipokines such as adiponectin and immune cells , especially macrophages , in adipose tissue .
	manualset3
256170	5	425904	7	NULL	NULL	NULL	NULL	immune cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current research is focused on the role of adipokines such as adiponectin and immune cells , especially macrophages , in adipose tissue .
	manualset3
256171	6	425904	7	NULL	NULL	NULL	NULL	macrophages	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current research is focused on the role of adipokines such as adiponectin and immune cells , especially macrophages , in adipose tissue .
	manualset3
256172	7	425904	7	NULL	NULL	NULL	NULL	adipose tissue	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current research is focused on the role of adipokines such as adiponectin and immune cells , especially macrophages , in adipose tissue .
	manualset3
256173	1	425905	7	NULL	NULL	NULL	NULL	Current status	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current status of urea-formaldehyde foam insulation .
	manualset3
256174	2	425905	7	NULL	NULL	NULL	NULL	urea-formaldehyde foam insulation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current status of urea-formaldehyde foam insulation .
	manualset3
256175	1	425906	7	NULL	NULL	NULL	NULL	Current strategies	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current strategies for the treatment of alcohol dependence in the United States .
	manualset3
256176	2	425906	7	NULL	NULL	NULL	NULL	treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current strategies for the treatment of alcohol dependence in the United States .
	manualset3
256178	3	425906	7	NULL	NULL	NULL	NULL	alcohol dependence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current strategies for the treatment of alcohol dependence in the United States .
	manualset3
256179	4	425906	7	NULL	NULL	NULL	NULL	United States	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current strategies for the treatment of alcohol dependence in the United States .
	manualset3
256180	1	425907	7	NULL	NULL	NULL	NULL	stroke prevention	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current stroke prevention focuses on optimizing the treatment of modifiable risk factors , such as hypertension , diabetes and dyslipidemia .
	manualset3
256181	2	425907	7	NULL	NULL	NULL	NULL	treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current stroke prevention focuses on optimizing the treatment of modifiable risk factors , such as hypertension , diabetes and dyslipidemia .
	manualset3
256182	3	425907	7	NULL	NULL	NULL	NULL	modifiable risk factors	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current stroke prevention focuses on optimizing the treatment of modifiable risk factors , such as hypertension , diabetes and dyslipidemia .
	manualset3
256183	4	425907	7	NULL	NULL	NULL	NULL	hypertension	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current stroke prevention focuses on optimizing the treatment of modifiable risk factors , such as hypertension , diabetes and dyslipidemia .
	manualset3
256184	5	425907	7	NULL	NULL	NULL	NULL	diabetes	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current stroke prevention focuses on optimizing the treatment of modifiable risk factors , such as hypertension , diabetes and dyslipidemia .
	manualset3
256185	6	425907	7	NULL	NULL	NULL	NULL	dyslipidemia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current stroke prevention focuses on optimizing the treatment of modifiable risk factors , such as hypertension , diabetes and dyslipidemia .
	manualset3
256186	1	425908	7	NULL	NULL	NULL	NULL	Current teaching opportunities	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current teaching and learning opportunities appear to be inadequate in their efforts to enhance and improve graduate nurses ' pharmacology knowledge .
	manualset3
256187	2	425908	7	NULL	NULL	NULL	NULL	 learning opportunities	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current teaching and learning opportunities appear to be inadequate in their efforts to enhance and improve graduate nurses ' pharmacology knowledge .
	manualset3
256188	3	425908	7	NULL	NULL	NULL	NULL	efforts 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current teaching and learning opportunities appear to be inadequate in their efforts to enhance and improve graduate nurses ' pharmacology knowledge .
	manualset3
256189	4	425908	7	NULL	NULL	NULL	NULL	graduate nurses '	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current teaching and learning opportunities appear to be inadequate in their efforts to enhance and improve graduate nurses ' pharmacology knowledge .
	manualset3
256190	5	425908	7	NULL	NULL	NULL	NULL	pharmacology knowledge	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current teaching and learning opportunities appear to be inadequate in their efforts to enhance and improve graduate nurses ' pharmacology knowledge .
	manualset3
256191	1	425909	7	NULL	NULL	NULL	NULL	 Megakaryoblastic leukemia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Megakaryoblastic leukemia and transient abnormal myelopoiesis with Down 's syndrome ) .
	manualset3
256192	2	425909	7	NULL	NULL	NULL	NULL	transient abnormal myelopoiesis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Megakaryoblastic leukemia and transient abnormal myelopoiesis with Down 's syndrome ) .
	manualset3
256193	3	425909	7	NULL	NULL	NULL	NULL	Down 's syndrome	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Megakaryoblastic leukemia and transient abnormal myelopoiesis with Down 's syndrome ) .
	manualset3
256194	1	425910	7	NULL	NULL	NULL	NULL	Current therapies	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current therapies are often inadequate to control elevated ICP in the clinical setting ( 5 , 6 , 7 ) .
	manualset3
256195	2	425910	7	NULL	NULL	NULL	NULL	elevated ICP	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current therapies are often inadequate to control elevated ICP in the clinical setting ( 5 , 6 , 7 ) .
	manualset3
256196	3	425910	7	NULL	NULL	NULL	NULL	clinical setting	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Current therapies are often inadequate to control elevated ICP in the clinical setting ( 5 , 6 , 7 ) .
	manualset3
256197	1	425911	7	NULL	NULL	NULL	NULL	several groups 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Currently , several groups are conducting clinical trials in cervix cancer , lung cancer , and brain tumors , using inhibitors of COX-2 in combination with chemotherapy and radiation therapy .
	manualset3
256198	2	425911	7	NULL	NULL	NULL	NULL	clinical trials	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Currently , several groups are conducting clinical trials in cervix cancer , lung cancer , and brain tumors , using inhibitors of COX-2 in combination with chemotherapy and radiation therapy .
	manualset3
256199	3	425911	7	NULL	NULL	NULL	NULL	cervix cancer	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Currently , several groups are conducting clinical trials in cervix cancer , lung cancer , and brain tumors , using inhibitors of COX-2 in combination with chemotherapy and radiation therapy .
	manualset3
256200	4	425911	7	NULL	NULL	NULL	NULL	 lung cancer	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Currently , several groups are conducting clinical trials in cervix cancer , lung cancer , and brain tumors , using inhibitors of COX-2 in combination with chemotherapy and radiation therapy .
	manualset3
256201	5	425911	7	NULL	NULL	NULL	NULL	brain tumors	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Currently , several groups are conducting clinical trials in cervix cancer , lung cancer , and brain tumors , using inhibitors of COX-2 in combination with chemotherapy and radiation therapy .
	manualset3
256202	6	425911	7	NULL	NULL	NULL	NULL	inhibitors	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Currently , several groups are conducting clinical trials in cervix cancer , lung cancer , and brain tumors , using inhibitors of COX-2 in combination with chemotherapy and radiation therapy .
	manualset3
256203	7	425911	7	NULL	NULL	NULL	NULL	COX-2 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Currently , several groups are conducting clinical trials in cervix cancer , lung cancer , and brain tumors , using inhibitors of COX-2 in combination with chemotherapy and radiation therapy .
	manualset3
256204	8	425911	7	NULL	NULL	NULL	NULL	combination	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Currently , several groups are conducting clinical trials in cervix cancer , lung cancer , and brain tumors , using inhibitors of COX-2 in combination with chemotherapy and radiation therapy .
	manualset3
256205	9	425911	7	NULL	NULL	NULL	NULL	chemotherapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Currently , several groups are conducting clinical trials in cervix cancer , lung cancer , and brain tumors , using inhibitors of COX-2 in combination with chemotherapy and radiation therapy .
	manualset3
256206	10	425911	7	NULL	NULL	NULL	NULL	radiation therapy 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Currently , several groups are conducting clinical trials in cervix cancer , lung cancer , and brain tumors , using inhibitors of COX-2 in combination with chemotherapy and radiation therapy .
	manualset3
256207	1	425912	7	NULL	NULL	NULL	NULL	` science-wikis '	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Currently , there are several such ` science-wikis ' that aim to collect specialist knowledge from the community into centralized resources .
	manualset3
256208	2	425912	7	NULL	NULL	NULL	NULL	specialist knowledge	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Currently , there are several such ` science-wikis ' that aim to collect specialist knowledge from the community into centralized resources .
	manualset3
256209	3	425912	7	NULL	NULL	NULL	NULL	 community	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Currently , there are several such ` science-wikis ' that aim to collect specialist knowledge from the community into centralized resources .
	manualset3
256210	4	425912	7	NULL	NULL	NULL	NULL	centralized resources	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Currently , there are several such ` science-wikis ' that aim to collect specialist knowledge from the community into centralized resources .
	manualset3
256211	1	425913	7	NULL	NULL	NULL	NULL	antidepressants	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Currently available antidepressants are known to affect the monoaminergic ( e.g. , serotonin , norepinephrine , and dopamine ) systems in the brain .
	manualset3
256212	2	425913	7	NULL	NULL	NULL	NULL	monoaminergic systems	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Currently available antidepressants are known to affect the monoaminergic ( e.g. , serotonin , norepinephrine , and dopamine ) systems in the brain .
	manualset3
256213	3	425913	7	NULL	NULL	NULL	NULL	serotonin	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Currently available antidepressants are known to affect the monoaminergic ( e.g. , serotonin , norepinephrine , and dopamine ) systems in the brain .
	manualset3
256214	4	425913	7	NULL	NULL	NULL	NULL	norepinephrine	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Currently available antidepressants are known to affect the monoaminergic ( e.g. , serotonin , norepinephrine , and dopamine ) systems in the brain .
	manualset3
256215	5	425913	7	NULL	NULL	NULL	NULL	dopamine	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Currently available antidepressants are known to affect the monoaminergic ( e.g. , serotonin , norepinephrine , and dopamine ) systems in the brain .
	manualset3
256216	6	425913	7	NULL	NULL	NULL	NULL	brain	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Currently available antidepressants are known to affect the monoaminergic ( e.g. , serotonin , norepinephrine , and dopamine ) systems in the brain .
	manualset3
256217	1	425914	7	NULL	NULL	NULL	NULL	Mental health 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Mental health and literature ) .
	manualset3
256218	2	425914	7	NULL	NULL	NULL	NULL	literature 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Mental health and literature ) .
	manualset3
256219	1	425915	7	NULL	NULL	NULL	NULL	Cutaneous metastases 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cutaneous metastases from colon cancer are uncommon and usually present as nodular lesions .
	manualset3
256220	2	425915	7	NULL	NULL	NULL	NULL	 colon cancer	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cutaneous metastases from colon cancer are uncommon and usually present as nodular lesions .
	manualset3
256221	3	425915	7	NULL	NULL	NULL	NULL	nodular lesions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cutaneous metastases from colon cancer are uncommon and usually present as nodular lesions .
	manualset3
256222	1	425916	7	NULL	NULL	NULL	NULL	Cyanamide	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyanamide was found to be essential for the formation of phosphatidylcholine , and only traces of HCl , of the order of that required to convert the disodium phosphatidate to free phosphatidic acid were found necessary for the synthesis .
	manualset3
256223	2	425916	7	NULL	NULL	NULL	NULL	 formation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyanamide was found to be essential for the formation of phosphatidylcholine , and only traces of HCl , of the order of that required to convert the disodium phosphatidate to free phosphatidic acid were found necessary for the synthesis .
	manualset3
256224	3	425916	7	NULL	NULL	NULL	NULL	phosphatidylcholine	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyanamide was found to be essential for the formation of phosphatidylcholine , and only traces of HCl , of the order of that required to convert the disodium phosphatidate to free phosphatidic acid were found necessary for the synthesis .
	manualset3
256225	4	425916	7	NULL	NULL	NULL	NULL	HCl	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyanamide was found to be essential for the formation of phosphatidylcholine , and only traces of HCl , of the order of that required to convert the disodium phosphatidate to free phosphatidic acid were found necessary for the synthesis .
	manualset3
256226	5	425916	7	NULL	NULL	NULL	NULL	order	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyanamide was found to be essential for the formation of phosphatidylcholine , and only traces of HCl , of the order of that required to convert the disodium phosphatidate to free phosphatidic acid were found necessary for the synthesis .
	manualset3
256227	6	425916	7	NULL	NULL	NULL	NULL	disodium phosphatidate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyanamide was found to be essential for the formation of phosphatidylcholine , and only traces of HCl , of the order of that required to convert the disodium phosphatidate to free phosphatidic acid were found necessary for the synthesis .
	manualset3
256228	7	425916	7	NULL	NULL	NULL	NULL	free phosphatidic acid	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyanamide was found to be essential for the formation of phosphatidylcholine , and only traces of HCl , of the order of that required to convert the disodium phosphatidate to free phosphatidic acid were found necessary for the synthesis .
	manualset3
256229	8	425916	7	NULL	NULL	NULL	NULL	synthesis	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyanamide was found to be essential for the formation of phosphatidylcholine , and only traces of HCl , of the order of that required to convert the disodium phosphatidate to free phosphatidic acid were found necessary for the synthesis .
	manualset3
256230	1	425917	7	NULL	NULL	NULL	NULL	Cyanobacterial cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyanobacterial cells and toxins from environmental bloom samples were more resistant to chlorination than results obtained using laboratory cultured cells and dissolved standard toxins .
	manualset3
256231	2	425917	7	NULL	NULL	NULL	NULL	toxins	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyanobacterial cells and toxins from environmental bloom samples were more resistant to chlorination than results obtained using laboratory cultured cells and dissolved standard toxins .
	manualset3
256232	3	425917	7	NULL	NULL	NULL	NULL	environmental bloom samples	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyanobacterial cells and toxins from environmental bloom samples were more resistant to chlorination than results obtained using laboratory cultured cells and dissolved standard toxins .
	manualset3
256233	4	425917	7	NULL	NULL	NULL	NULL	chlorination	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyanobacterial cells and toxins from environmental bloom samples were more resistant to chlorination than results obtained using laboratory cultured cells and dissolved standard toxins .
	manualset3
256234	5	425917	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyanobacterial cells and toxins from environmental bloom samples were more resistant to chlorination than results obtained using laboratory cultured cells and dissolved standard toxins .
	manualset3
256235	6	425917	7	NULL	NULL	NULL	NULL	laboratory cultured cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyanobacterial cells and toxins from environmental bloom samples were more resistant to chlorination than results obtained using laboratory cultured cells and dissolved standard toxins .
	manualset3
256236	7	425917	7	NULL	NULL	NULL	NULL	standard toxins	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyanobacterial cells and toxins from environmental bloom samples were more resistant to chlorination than results obtained using laboratory cultured cells and dissolved standard toxins .
	manualset3
256237	1	425918	7	NULL	NULL	NULL	NULL	Cycle sequencing reactions	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cycle sequencing reactions using Applied Biosystems BigDye ( ) Terminator Ready Reaction v1 .1 or v3 .1 Kit are performed , then purification of sequence reactions before electrophoresing using Applied Biosystems 3730 or 3730XL Genetic Analyser ( or similar ) .
	manualset3
256238	2	425918	7	NULL	NULL	NULL	NULL	Applied Biosystems BigDye ( ) Terminator Ready Reaction v1 .1	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cycle sequencing reactions using Applied Biosystems BigDye ( ) Terminator Ready Reaction v1 .1 or v3 .1 Kit are performed , then purification of sequence reactions before electrophoresing using Applied Biosystems 3730 or 3730XL Genetic Analyser ( or similar ) .
	manualset3
256240	4	425918	7	NULL	NULL	NULL	NULL	 v3 .1 Kit	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cycle sequencing reactions using Applied Biosystems BigDye ( ) Terminator Ready Reaction v1 .1 or v3 .1 Kit are performed , then purification of sequence reactions before electrophoresing using Applied Biosystems 3730 or 3730XL Genetic Analyser ( or similar ) .
	manualset3
256241	5	425918	7	NULL	NULL	NULL	NULL	purification	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cycle sequencing reactions using Applied Biosystems BigDye ( ) Terminator Ready Reaction v1 .1 or v3 .1 Kit are performed , then purification of sequence reactions before electrophoresing using Applied Biosystems 3730 or 3730XL Genetic Analyser ( or similar ) .
	manualset3
256242	6	425918	7	NULL	NULL	NULL	NULL	sequence reactions	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cycle sequencing reactions using Applied Biosystems BigDye ( ) Terminator Ready Reaction v1 .1 or v3 .1 Kit are performed , then purification of sequence reactions before electrophoresing using Applied Biosystems 3730 or 3730XL Genetic Analyser ( or similar ) .
	manualset3
256243	7	425918	7	NULL	NULL	NULL	NULL	Applied Biosystems 3730	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cycle sequencing reactions using Applied Biosystems BigDye ( ) Terminator Ready Reaction v1 .1 or v3 .1 Kit are performed , then purification of sequence reactions before electrophoresing using Applied Biosystems 3730 or 3730XL Genetic Analyser ( or similar ) .
	manualset3
256244	8	425918	7	NULL	NULL	NULL	NULL	 3730XL Genetic Analyser 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cycle sequencing reactions using Applied Biosystems BigDye ( ) Terminator Ready Reaction v1 .1 or v3 .1 Kit are performed , then purification of sequence reactions before electrophoresing using Applied Biosystems 3730 or 3730XL Genetic Analyser ( or similar ) .
	manualset3
256245	1	425919	7	NULL	NULL	NULL	NULL	Cyclic ADP-ribose	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic ADP-ribose and the regulation of calcium-induced calcium release in eggs and cardiac myocytes .
	manualset3
256246	2	425919	7	NULL	NULL	NULL	NULL	regulation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic ADP-ribose and the regulation of calcium-induced calcium release in eggs and cardiac myocytes .
	manualset3
256247	3	425919	7	NULL	NULL	NULL	NULL	calcium-induced calcium release	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic ADP-ribose and the regulation of calcium-induced calcium release in eggs and cardiac myocytes .
	manualset3
256248	4	425919	7	NULL	NULL	NULL	NULL	eggs	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic ADP-ribose and the regulation of calcium-induced calcium release in eggs and cardiac myocytes .
	manualset3
256249	5	425919	7	NULL	NULL	NULL	NULL	cardiac myocytes	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic ADP-ribose and the regulation of calcium-induced calcium release in eggs and cardiac myocytes .
	manualset3
256250	1	425920	7	NULL	NULL	NULL	NULL	Cyclic AMP-independent protein kinase activities	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic AMP-independent protein kinase activities from Ehrlich ascites tumor cells , partially purified by DEAE-cellulose and phosphocellulose chromatography were inhibited by quercetin .
	manualset3
256251	2	425920	7	NULL	NULL	NULL	NULL	Ehrlich ascites tumor cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic AMP-independent protein kinase activities from Ehrlich ascites tumor cells , partially purified by DEAE-cellulose and phosphocellulose chromatography were inhibited by quercetin .
	manualset3
256252	3	425920	7	NULL	NULL	NULL	NULL	DEAE-cellulose	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic AMP-independent protein kinase activities from Ehrlich ascites tumor cells , partially purified by DEAE-cellulose and phosphocellulose chromatography were inhibited by quercetin .
	manualset3
256253	4	425920	7	NULL	NULL	NULL	NULL	phosphocellulose chromatography	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic AMP-independent protein kinase activities from Ehrlich ascites tumor cells , partially purified by DEAE-cellulose and phosphocellulose chromatography were inhibited by quercetin .
	manualset3
256254	5	425920	7	NULL	NULL	NULL	NULL	quercetin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic AMP-independent protein kinase activities from Ehrlich ascites tumor cells , partially purified by DEAE-cellulose and phosphocellulose chromatography were inhibited by quercetin .
	manualset3
256255	1	425921	7	NULL	NULL	NULL	NULL	Cyclic AMP	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic AMP in mycobacteria : characterization and functional role of the Rv1647 ortholog in Mycobacterium smegmatis .
	manualset3
256256	2	425921	7	NULL	NULL	NULL	NULL	mycobacteria	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic AMP in mycobacteria : characterization and functional role of the Rv1647 ortholog in Mycobacterium smegmatis .
	manualset3
256257	3	425921	7	NULL	NULL	NULL	NULL	 characterization 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic AMP in mycobacteria : characterization and functional role of the Rv1647 ortholog in Mycobacterium smegmatis .
	manualset3
256258	4	425921	7	NULL	NULL	NULL	NULL	functional role	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic AMP in mycobacteria : characterization and functional role of the Rv1647 ortholog in Mycobacterium smegmatis .
	manualset3
256259	5	425921	7	NULL	NULL	NULL	NULL	Rv1647 ortholog	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic AMP in mycobacteria : characterization and functional role of the Rv1647 ortholog in Mycobacterium smegmatis .
	manualset3
256260	6	425921	7	NULL	NULL	NULL	NULL	Mycobacterium smegmatis	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic AMP in mycobacteria : characterization and functional role of the Rv1647 ortholog in Mycobacterium smegmatis .
	manualset3
256261	1	425922	7	NULL	NULL	NULL	NULL	Method 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Method and meaning research on skin-test of four injections of traditional Chinese medicine ) .
	manualset3
256262	2	425922	7	NULL	NULL	NULL	NULL	research	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Method and meaning research on skin-test of four injections of traditional Chinese medicine ) .
	manualset3
256263	3	425922	7	NULL	NULL	NULL	NULL	skin-test 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Method and meaning research on skin-test of four injections of traditional Chinese medicine ) .
	manualset3
256264	4	425922	7	NULL	NULL	NULL	NULL	four injections	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Method and meaning research on skin-test of four injections of traditional Chinese medicine ) .
	manualset3
256265	5	425922	7	NULL	NULL	NULL	NULL	 traditional Chinese medicine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Method and meaning research on skin-test of four injections of traditional Chinese medicine ) .
	manualset3
256266	1	425923	7	NULL	NULL	NULL	NULL	Cyclic AMP levels	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic AMP levels increased with the size of burn .
	manualset3
256267	2	425923	7	NULL	NULL	NULL	NULL	size	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic AMP levels increased with the size of burn .
	manualset3
256268	3	425923	7	NULL	NULL	NULL	NULL	 burn	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic AMP levels increased with the size of burn .
	manualset3
256269	1	425924	7	NULL	NULL	NULL	NULL	Cyclic nucleotides	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic nucleotides in heart in acute myocardial ischemia and hypoxia .
	manualset3
256270	2	425924	7	NULL	NULL	NULL	NULL	heart	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic nucleotides in heart in acute myocardial ischemia and hypoxia .
	manualset3
256271	3	425924	7	NULL	NULL	NULL	NULL	 acute myocardial ischemia 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic nucleotides in heart in acute myocardial ischemia and hypoxia .
	manualset3
256272	4	425924	7	NULL	NULL	NULL	NULL	hypoxia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic nucleotides in heart in acute myocardial ischemia and hypoxia .
	manualset3
256526	1	425925	7	NULL	NULL	NULL	NULL	Cyclic psychosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic psychosis , menstrual cycle and adolescence .
	manualset3
256527	2	425925	7	NULL	NULL	NULL	NULL	menstrual cycle 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic psychosis , menstrual cycle and adolescence .
	manualset3
256528	3	425925	7	NULL	NULL	NULL	NULL	adolescence	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic psychosis , menstrual cycle and adolescence .
	manualset3
256530	1	425926	7	NULL	NULL	NULL	NULL	Cyclic voltammetric experiments	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic voltammetric experiments in CH ( 2 ) Cl ( 2 ) reveal quasireversible Co ( III ) - Co ( II ) , Ni ( III ) - Ni ( II ) and Cu ( II ) - Cu ( I ) redox processes .
	manualset3
256532	2	425926	7	NULL	NULL	NULL	NULL	CH ( 2 ) Cl ( 2 )	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic voltammetric experiments in CH ( 2 ) Cl ( 2 ) reveal quasireversible Co ( III ) - Co ( II ) , Ni ( III ) - Ni ( II ) and Cu ( II ) - Cu ( I ) redox processes .
	manualset3
256533	3	425926	7	NULL	NULL	NULL	NULL	quasireversible Co ( III ) - Co ( II ) redox processes	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic voltammetric experiments in CH ( 2 ) Cl ( 2 ) reveal quasireversible Co ( III ) - Co ( II ) , Ni ( III ) - Ni ( II ) and Cu ( II ) - Cu ( I ) redox processes .
	manualset3
256539	4	425926	7	NULL	NULL	NULL	NULL	Ni ( III ) - Ni ( II ) redox processes	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic voltammetric experiments in CH ( 2 ) Cl ( 2 ) reveal quasireversible Co ( III ) - Co ( II ) , Ni ( III ) - Ni ( II ) and Cu ( II ) - Cu ( I ) redox processes .
	manualset3
256540	5	425926	7	NULL	NULL	NULL	NULL	Cu ( II ) - Cu ( I ) redox processes	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclic voltammetric experiments in CH ( 2 ) Cl ( 2 ) reveal quasireversible Co ( III ) - Co ( II ) , Ni ( III ) - Ni ( II ) and Cu ( II ) - Cu ( I ) redox processes .
	manualset3
256545	1	425927	7	NULL	NULL	NULL	NULL	Cyclical etidronate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclical etidronate and calcium carbonate ( with citrate ) supplementation for osteoporosis unmasking primary hyperparathyroidism .
	manualset3
256546	2	425927	7	NULL	NULL	NULL	NULL	calcium carbonate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclical etidronate and calcium carbonate ( with citrate ) supplementation for osteoporosis unmasking primary hyperparathyroidism .
	manualset3
256548	3	425927	7	NULL	NULL	NULL	NULL	citrate 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclical etidronate and calcium carbonate ( with citrate ) supplementation for osteoporosis unmasking primary hyperparathyroidism .
	manualset3
256549	4	425927	7	NULL	NULL	NULL	NULL	supplementation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclical etidronate and calcium carbonate ( with citrate ) supplementation for osteoporosis unmasking primary hyperparathyroidism .
	manualset3
256552	5	425927	7	NULL	NULL	NULL	NULL	osteoporosis unmasking primary hyperparathyroidism	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclical etidronate and calcium carbonate ( with citrate ) supplementation for osteoporosis unmasking primary hyperparathyroidism .
	manualset3
256554	1	425928	7	NULL	NULL	NULL	NULL	Cyclin-dependent kinases ( Cdks )	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclin-dependent kinases ( Cdks ) are a family of proline-directed Ser/Thr kinases known for their role in the control of cell cycle progression .
	manualset3
256556	2	425928	7	NULL	NULL	NULL	NULL	 family	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclin-dependent kinases ( Cdks ) are a family of proline-directed Ser/Thr kinases known for their role in the control of cell cycle progression .
	manualset3
256558	3	425928	7	NULL	NULL	NULL	NULL	proline-directed Ser/Thr kinases	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclin-dependent kinases ( Cdks ) are a family of proline-directed Ser/Thr kinases known for their role in the control of cell cycle progression .
	manualset3
256561	4	425928	7	NULL	NULL	NULL	NULL	role	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclin-dependent kinases ( Cdks ) are a family of proline-directed Ser/Thr kinases known for their role in the control of cell cycle progression .
	manualset3
256563	5	425928	7	NULL	NULL	NULL	NULL	control	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclin-dependent kinases ( Cdks ) are a family of proline-directed Ser/Thr kinases known for their role in the control of cell cycle progression .
	manualset3
256565	6	425928	7	NULL	NULL	NULL	NULL	cell cycle progression	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclin-dependent kinases ( Cdks ) are a family of proline-directed Ser/Thr kinases known for their role in the control of cell cycle progression .
	manualset3
256572	1	425929	7	NULL	NULL	NULL	NULL	Cyclin D1 ( CyD1 )	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclin D1 ( CyD1 ) is a pivotal cell cycle-regulatory molecule and a well-studied therapeutic target for cancer .
	manualset3
256574	2	425929	7	NULL	NULL	NULL	NULL	cell cycle-regulatory molecule	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclin D1 ( CyD1 ) is a pivotal cell cycle-regulatory molecule and a well-studied therapeutic target for cancer .
	manualset3
256575	3	425929	7	NULL	NULL	NULL	NULL	therapeutic target 	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclin D1 ( CyD1 ) is a pivotal cell cycle-regulatory molecule and a well-studied therapeutic target for cancer .
	manualset3
256576	4	425929	7	NULL	NULL	NULL	NULL	cancer	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclin D1 ( CyD1 ) is a pivotal cell cycle-regulatory molecule and a well-studied therapeutic target for cancer .
	manualset3
256579	1	425930	7	NULL	NULL	NULL	NULL	Cyclin D2	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclin D2 , a member of the D-type cyclins , implicated in cell cycle regulation , differentiation and malignant transformation , is inactivated due to aberrant DNA methylation in several human cancers .
	manualset3
256581	2	425930	7	NULL	NULL	NULL	NULL	 member 	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclin D2 , a member of the D-type cyclins , implicated in cell cycle regulation , differentiation and malignant transformation , is inactivated due to aberrant DNA methylation in several human cancers .
	manualset3
256582	3	425930	7	NULL	NULL	NULL	NULL	D-type cyclins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclin D2 , a member of the D-type cyclins , implicated in cell cycle regulation , differentiation and malignant transformation , is inactivated due to aberrant DNA methylation in several human cancers .
	manualset3
256584	4	425930	7	NULL	NULL	NULL	NULL	cell cycle regulation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclin D2 , a member of the D-type cyclins , implicated in cell cycle regulation , differentiation and malignant transformation , is inactivated due to aberrant DNA methylation in several human cancers .
	manualset3
256585	5	425930	7	NULL	NULL	NULL	NULL	differentiation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclin D2 , a member of the D-type cyclins , implicated in cell cycle regulation , differentiation and malignant transformation , is inactivated due to aberrant DNA methylation in several human cancers .
	manualset3
256586	6	425930	7	NULL	NULL	NULL	NULL	malignant transformation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclin D2 , a member of the D-type cyclins , implicated in cell cycle regulation , differentiation and malignant transformation , is inactivated due to aberrant DNA methylation in several human cancers .
	manualset3
256588	7	425930	7	NULL	NULL	NULL	NULL	aberrant DNA methylation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclin D2 , a member of the D-type cyclins , implicated in cell cycle regulation , differentiation and malignant transformation , is inactivated due to aberrant DNA methylation in several human cancers .
	manualset3
256589	8	425930	7	NULL	NULL	NULL	NULL	human cancers	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclin D2 , a member of the D-type cyclins , implicated in cell cycle regulation , differentiation and malignant transformation , is inactivated due to aberrant DNA methylation in several human cancers .
	manualset3
256594	1	425931	7	NULL	NULL	NULL	NULL	Cycloheximide	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cycloheximide had no affect on basal or insulin-stimulated 3-O-methylglucose uptake in intact cells or in plasma membrane vesicles .
	manualset3
256595	2	425931	7	NULL	NULL	NULL	NULL	 affect	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cycloheximide had no affect on basal or insulin-stimulated 3-O-methylglucose uptake in intact cells or in plasma membrane vesicles .
	manualset3
256596	3	425931	7	NULL	NULL	NULL	NULL	 basal uptake	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cycloheximide had no affect on basal or insulin-stimulated 3-O-methylglucose uptake in intact cells or in plasma membrane vesicles .
	manualset3
256597	4	425931	7	NULL	NULL	NULL	NULL	insulin-stimulated 3-O-methylglucose uptake	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cycloheximide had no affect on basal or insulin-stimulated 3-O-methylglucose uptake in intact cells or in plasma membrane vesicles .
	manualset3
256598	5	425931	7	NULL	NULL	NULL	NULL	intact cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cycloheximide had no affect on basal or insulin-stimulated 3-O-methylglucose uptake in intact cells or in plasma membrane vesicles .
	manualset3
256599	6	425931	7	NULL	NULL	NULL	NULL	plasma membrane vesicles	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cycloheximide had no affect on basal or insulin-stimulated 3-O-methylglucose uptake in intact cells or in plasma membrane vesicles .
	manualset3
257038	1	425932	7	NULL	NULL	NULL	NULL	Cyclophilin-40	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclophilin-40 has a cellular role in the aryl hydrocarbon receptor signaling .
	manualset3
257039	2	425932	7	NULL	NULL	NULL	NULL	cellular role	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclophilin-40 has a cellular role in the aryl hydrocarbon receptor signaling .
	manualset3
257040	3	425932	7	NULL	NULL	NULL	NULL	aryl hydrocarbon receptor signaling	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclophilin-40 has a cellular role in the aryl hydrocarbon receptor signaling .
	manualset3
257041	1	425933	7	NULL	NULL	NULL	NULL	Cyclosporin A 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclosporin A decreased the rate of choline transport but not the binding of the non-transportable choline analog hemicholinium-3 , indicating that the number of membrane transporters was not affected .
	manualset3
257042	2	425933	7	NULL	NULL	NULL	NULL	rate	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclosporin A decreased the rate of choline transport but not the binding of the non-transportable choline analog hemicholinium-3 , indicating that the number of membrane transporters was not affected .
	manualset3
257043	3	425933	7	NULL	NULL	NULL	NULL	choline transport 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclosporin A decreased the rate of choline transport but not the binding of the non-transportable choline analog hemicholinium-3 , indicating that the number of membrane transporters was not affected .
	manualset3
257044	4	425933	7	NULL	NULL	NULL	NULL	binding 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclosporin A decreased the rate of choline transport but not the binding of the non-transportable choline analog hemicholinium-3 , indicating that the number of membrane transporters was not affected .
	manualset3
257045	5	425933	7	NULL	NULL	NULL	NULL	non-transportable choline analog	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclosporin A decreased the rate of choline transport but not the binding of the non-transportable choline analog hemicholinium-3 , indicating that the number of membrane transporters was not affected .
	manualset3
257046	6	425933	7	NULL	NULL	NULL	NULL	hemicholinium-3	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclosporin A decreased the rate of choline transport but not the binding of the non-transportable choline analog hemicholinium-3 , indicating that the number of membrane transporters was not affected .
	manualset3
257047	7	425933	7	NULL	NULL	NULL	NULL	number	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclosporin A decreased the rate of choline transport but not the binding of the non-transportable choline analog hemicholinium-3 , indicating that the number of membrane transporters was not affected .
	manualset3
257048	8	425933	7	NULL	NULL	NULL	NULL	membrane transporters	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclosporin A decreased the rate of choline transport but not the binding of the non-transportable choline analog hemicholinium-3 , indicating that the number of membrane transporters was not affected .
	manualset3
257088	1	425934	7	NULL	NULL	NULL	NULL	Cyclosporin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclosporin and quinidine inhibition of renal digoxin excretion : evidence for luminal secretion of digoxin .
	manualset3
257089	2	425934	7	NULL	NULL	NULL	NULL	quinidine inhibition	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclosporin and quinidine inhibition of renal digoxin excretion : evidence for luminal secretion of digoxin .
	manualset3
257090	3	425934	7	NULL	NULL	NULL	NULL	renal digoxin excretion	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclosporin and quinidine inhibition of renal digoxin excretion : evidence for luminal secretion of digoxin .
	manualset3
257091	4	425934	7	NULL	NULL	NULL	NULL	evidence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclosporin and quinidine inhibition of renal digoxin excretion : evidence for luminal secretion of digoxin .
	manualset3
257092	5	425934	7	NULL	NULL	NULL	NULL	 luminal secretion	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclosporin and quinidine inhibition of renal digoxin excretion : evidence for luminal secretion of digoxin .
	manualset3
257093	6	425934	7	NULL	NULL	NULL	NULL	digoxin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclosporin and quinidine inhibition of renal digoxin excretion : evidence for luminal secretion of digoxin .
	manualset3
257094	1	425935	7	NULL	NULL	NULL	NULL	Cyclosporine treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclosporine treatment reduces oxygen free radical generation and oxidative stress in the brain of hypoxia-reoxygenated newborn piglets .
	manualset3
257095	2	425935	7	NULL	NULL	NULL	NULL	oxygen free radical generation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclosporine treatment reduces oxygen free radical generation and oxidative stress in the brain of hypoxia-reoxygenated newborn piglets .
	manualset3
257096	3	425935	7	NULL	NULL	NULL	NULL	oxidative stress	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclosporine treatment reduces oxygen free radical generation and oxidative stress in the brain of hypoxia-reoxygenated newborn piglets .
	manualset3
257097	4	425935	7	NULL	NULL	NULL	NULL	brain 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclosporine treatment reduces oxygen free radical generation and oxidative stress in the brain of hypoxia-reoxygenated newborn piglets .
	manualset3
257098	5	425935	7	NULL	NULL	NULL	NULL	hypoxia-reoxygenated newborn piglets	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cyclosporine treatment reduces oxygen free radical generation and oxidative stress in the brain of hypoxia-reoxygenated newborn piglets .
	manualset3
257099	1	425936	7	NULL	NULL	NULL	NULL	Cylindrical sources	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cylindrical sources are used in the calibration process placed perpendicularly to the detector 's axis .
	manualset3
257100	2	425936	7	NULL	NULL	NULL	NULL	calibration process	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cylindrical sources are used in the calibration process placed perpendicularly to the detector 's axis .
	manualset3
257101	3	425936	7	NULL	NULL	NULL	NULL	 detector 's axis	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cylindrical sources are used in the calibration process placed perpendicularly to the detector 's axis .
	manualset3
257102	1	425937	7	NULL	NULL	NULL	NULL	Cynomolgus monkeys	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cynomolgus monkeys were fed an atherogenic diet that produces both hypercholesterolemia and moderate hyperhomocyst ( e ) inemia .
	manualset3
257103	2	425937	7	NULL	NULL	NULL	NULL	atherogenic diet	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cynomolgus monkeys were fed an atherogenic diet that produces both hypercholesterolemia and moderate hyperhomocyst ( e ) inemia .
	manualset3
257104	3	425937	7	NULL	NULL	NULL	NULL	 hypercholesterolemia 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cynomolgus monkeys were fed an atherogenic diet that produces both hypercholesterolemia and moderate hyperhomocyst ( e ) inemia .
	manualset3
257105	4	425937	7	NULL	NULL	NULL	NULL	hyperhomocyst ( e ) inemia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cynomolgus monkeys were fed an atherogenic diet that produces both hypercholesterolemia and moderate hyperhomocyst ( e ) inemia .
	manualset3
257106	1	425938	7	NULL	NULL	NULL	NULL	Cystathionine beta synthase deficiency	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cystathionine beta synthase deficiency induces hyperhomocysteinemia which is considered as a risk factor for vascular diseases .
	manualset3
257107	2	425938	7	NULL	NULL	NULL	NULL	hyperhomocysteinemia 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cystathionine beta synthase deficiency induces hyperhomocysteinemia which is considered as a risk factor for vascular diseases .
	manualset3
257108	3	425938	7	NULL	NULL	NULL	NULL	 risk factor	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cystathionine beta synthase deficiency induces hyperhomocysteinemia which is considered as a risk factor for vascular diseases .
	manualset3
257109	4	425938	7	NULL	NULL	NULL	NULL	vascular diseases	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cystathionine beta synthase deficiency induces hyperhomocysteinemia which is considered as a risk factor for vascular diseases .
	manualset3
257110	1	425939	7	NULL	NULL	NULL	NULL	Cystatin C	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cystatin C is an amyloidogenic protein that colocalizes with beta-amyloid ( Abeta ) within arteriolar walls in Alzheimer disease ( AD ) brains .
	manualset3
257111	2	425939	7	NULL	NULL	NULL	NULL	amyloidogenic protein	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cystatin C is an amyloidogenic protein that colocalizes with beta-amyloid ( Abeta ) within arteriolar walls in Alzheimer disease ( AD ) brains .
	manualset3
257112	3	425939	7	NULL	NULL	NULL	NULL	beta-amyloid ( Abeta )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cystatin C is an amyloidogenic protein that colocalizes with beta-amyloid ( Abeta ) within arteriolar walls in Alzheimer disease ( AD ) brains .
	manualset3
257113	4	425939	7	NULL	NULL	NULL	NULL	arteriolar walls	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cystatin C is an amyloidogenic protein that colocalizes with beta-amyloid ( Abeta ) within arteriolar walls in Alzheimer disease ( AD ) brains .
	manualset3
257114	5	425939	7	NULL	NULL	NULL	NULL	Alzheimer disease ( AD ) brains	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cystatin C is an amyloidogenic protein that colocalizes with beta-amyloid ( Abeta ) within arteriolar walls in Alzheimer disease ( AD ) brains .
	manualset3
257115	1	425940	7	NULL	NULL	NULL	NULL	Cysteamine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cysteamine given subcutaneously in doses of 100-300 mg/kg , decreased the level of arterial blood glucose dose dependently , but had no effects on the level of the jugular venous blood glucose .
	manualset3
257116	2	425940	7	NULL	NULL	NULL	NULL	doses	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cysteamine given subcutaneously in doses of 100-300 mg/kg , decreased the level of arterial blood glucose dose dependently , but had no effects on the level of the jugular venous blood glucose .
	manualset3
257117	3	425940	7	NULL	NULL	NULL	NULL	100-300 mg/kg	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cysteamine given subcutaneously in doses of 100-300 mg/kg , decreased the level of arterial blood glucose dose dependently , but had no effects on the level of the jugular venous blood glucose .
	manualset3
257118	4	425940	7	NULL	NULL	NULL	NULL	level	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cysteamine given subcutaneously in doses of 100-300 mg/kg , decreased the level of arterial blood glucose dose dependently , but had no effects on the level of the jugular venous blood glucose .
	manualset3
257119	5	425940	7	NULL	NULL	NULL	NULL	arterial blood glucose dose	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cysteamine given subcutaneously in doses of 100-300 mg/kg , decreased the level of arterial blood glucose dose dependently , but had no effects on the level of the jugular venous blood glucose .
	manualset3
257120	6	425940	7	NULL	NULL	NULL	NULL	 effects	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cysteamine given subcutaneously in doses of 100-300 mg/kg , decreased the level of arterial blood glucose dose dependently , but had no effects on the level of the jugular venous blood glucose .
	manualset3
257121	7	425940	7	NULL	NULL	NULL	NULL	 level	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cysteamine given subcutaneously in doses of 100-300 mg/kg , decreased the level of arterial blood glucose dose dependently , but had no effects on the level of the jugular venous blood glucose .
	manualset3
257122	8	425940	7	NULL	NULL	NULL	NULL	jugular venous blood glucose	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cysteamine given subcutaneously in doses of 100-300 mg/kg , decreased the level of arterial blood glucose dose dependently , but had no effects on the level of the jugular venous blood glucose .
	manualset3
257123	1	425941	7	NULL	NULL	NULL	NULL	Cystein 402	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cystein 402 of HIV gp 120 is essential for CD4-binding and resistance of gp 120 to intracellular degradation .
	manualset3
257124	2	425941	7	NULL	NULL	NULL	NULL	HIV gp 120 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cystein 402 of HIV gp 120 is essential for CD4-binding and resistance of gp 120 to intracellular degradation .
	manualset3
257125	3	425941	7	NULL	NULL	NULL	NULL	CD4-binding	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cystein 402 of HIV gp 120 is essential for CD4-binding and resistance of gp 120 to intracellular degradation .
	manualset3
257126	4	425941	7	NULL	NULL	NULL	NULL	resistance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cystein 402 of HIV gp 120 is essential for CD4-binding and resistance of gp 120 to intracellular degradation .
	manualset3
257127	5	425941	7	NULL	NULL	NULL	NULL	gp 120	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cystein 402 of HIV gp 120 is essential for CD4-binding and resistance of gp 120 to intracellular degradation .
	manualset3
257128	6	425941	7	NULL	NULL	NULL	NULL	intracellular degradation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cystein 402 of HIV gp 120 is essential for CD4-binding and resistance of gp 120 to intracellular degradation .
	manualset3
257129	1	425942	7	NULL	NULL	NULL	NULL	Cysteine desulfurases	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cysteine desulfurases , such as yeast NFS1 , are required for sulfur addition to iron-sulfur clusters and other sulfur-requiring processes .
	manualset3
257130	2	425942	7	NULL	NULL	NULL	NULL	yeast NFS1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cysteine desulfurases , such as yeast NFS1 , are required for sulfur addition to iron-sulfur clusters and other sulfur-requiring processes .
	manualset3
257131	3	425942	7	NULL	NULL	NULL	NULL	sulfur addition	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cysteine desulfurases , such as yeast NFS1 , are required for sulfur addition to iron-sulfur clusters and other sulfur-requiring processes .
	manualset3
257132	4	425942	7	NULL	NULL	NULL	NULL	 iron-sulfur clusters	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cysteine desulfurases , such as yeast NFS1 , are required for sulfur addition to iron-sulfur clusters and other sulfur-requiring processes .
	manualset3
257133	5	425942	7	NULL	NULL	NULL	NULL	sulfur-requiring processes	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cysteine desulfurases , such as yeast NFS1 , are required for sulfur addition to iron-sulfur clusters and other sulfur-requiring processes .
	manualset3
257134	1	425943	7	NULL	NULL	NULL	NULL	Cystography 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cystography was carried out in 38 out of 54 patients to exclude bladder trauma .
	manualset3
257135	2	425943	7	NULL	NULL	NULL	NULL	38 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cystography was carried out in 38 out of 54 patients to exclude bladder trauma .
	manualset3
257136	3	425943	7	NULL	NULL	NULL	NULL	54 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cystography was carried out in 38 out of 54 patients to exclude bladder trauma .
	manualset3
257137	4	425943	7	NULL	NULL	NULL	NULL	bladder trauma	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cystography was carried out in 38 out of 54 patients to exclude bladder trauma .
	manualset3
257138	1	425944	7	NULL	NULL	NULL	NULL	Cytochalasin B ( CB ) 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochalasin B ( CB ) , a mold metabolite that inhibits various types of cell motility , has a dose-dependent inhibitory effect on the uptake of sucrose - ( 3 ) H by these cells .
	manualset3
257139	2	425944	7	NULL	NULL	NULL	NULL	 mold metabolite	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochalasin B ( CB ) , a mold metabolite that inhibits various types of cell motility , has a dose-dependent inhibitory effect on the uptake of sucrose - ( 3 ) H by these cells .
	manualset3
257140	4	425944	7	NULL	NULL	NULL	NULL	cell motility	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochalasin B ( CB ) , a mold metabolite that inhibits various types of cell motility , has a dose-dependent inhibitory effect on the uptake of sucrose - ( 3 ) H by these cells .
	manualset3
257141	3	425944	7	NULL	NULL	NULL	NULL	various types	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochalasin B ( CB ) , a mold metabolite that inhibits various types of cell motility , has a dose-dependent inhibitory effect on the uptake of sucrose - ( 3 ) H by these cells .
	manualset3
257142	5	425944	7	NULL	NULL	NULL	NULL	dose-dependent inhibitory effect 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochalasin B ( CB ) , a mold metabolite that inhibits various types of cell motility , has a dose-dependent inhibitory effect on the uptake of sucrose - ( 3 ) H by these cells .
	manualset3
257143	6	425944	7	NULL	NULL	NULL	NULL	uptake	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochalasin B ( CB ) , a mold metabolite that inhibits various types of cell motility , has a dose-dependent inhibitory effect on the uptake of sucrose - ( 3 ) H by these cells .
	manualset3
257144	7	425944	7	NULL	NULL	NULL	NULL	sucrose - ( 3 ) H 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochalasin B ( CB ) , a mold metabolite that inhibits various types of cell motility , has a dose-dependent inhibitory effect on the uptake of sucrose - ( 3 ) H by these cells .
	manualset3
257145	8	425944	7	NULL	NULL	NULL	NULL	cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochalasin B ( CB ) , a mold metabolite that inhibits various types of cell motility , has a dose-dependent inhibitory effect on the uptake of sucrose - ( 3 ) H by these cells .
	manualset3
257146	1	425945	7	NULL	NULL	NULL	NULL	Cytochalasin D ( CD ) 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochalasin D ( CD ) , an inhibitor of phagocytosis , blocked LPS internalization .
	manualset3
257147	2	425945	7	NULL	NULL	NULL	NULL	inhibitor	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochalasin D ( CD ) , an inhibitor of phagocytosis , blocked LPS internalization .
	manualset3
257148	3	425945	7	NULL	NULL	NULL	NULL	phagocytosis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochalasin D ( CD ) , an inhibitor of phagocytosis , blocked LPS internalization .
	manualset3
257149	4	425945	7	NULL	NULL	NULL	NULL	LPS internalization	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochalasin D ( CD ) , an inhibitor of phagocytosis , blocked LPS internalization .
	manualset3
257150	1	425946	7	NULL	NULL	NULL	NULL	Cytochemistry	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochemistry of leukocytic enzymes in Down 's syndrome .
	manualset3
257151	2	425946	7	NULL	NULL	NULL	NULL	leukocytic enzymes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochemistry of leukocytic enzymes in Down 's syndrome .
	manualset3
257152	3	425946	7	NULL	NULL	NULL	NULL	Down 's syndrome 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochemistry of leukocytic enzymes in Down 's syndrome .
	manualset3
257153	1	425947	7	NULL	NULL	NULL	NULL	Cytochrome C	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochrome C in a dry trehalose matrix : structural and dynamical effects probed by x-ray absorption spectroscopy .
	manualset3
257154	2	425947	7	NULL	NULL	NULL	NULL	 dry trehalose matrix	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochrome C in a dry trehalose matrix : structural and dynamical effects probed by x-ray absorption spectroscopy .
	manualset3
257155	3	425947	7	NULL	NULL	NULL	NULL	structural effects	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochrome C in a dry trehalose matrix : structural and dynamical effects probed by x-ray absorption spectroscopy .
	manualset3
257156	4	425947	7	NULL	NULL	NULL	NULL	dynamical effects	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochrome C in a dry trehalose matrix : structural and dynamical effects probed by x-ray absorption spectroscopy .
	manualset3
257157	5	425947	7	NULL	NULL	NULL	NULL	 x-ray absorption spectroscopy	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochrome C in a dry trehalose matrix : structural and dynamical effects probed by x-ray absorption spectroscopy .
	manualset3
257158	1	425948	7	NULL	NULL	NULL	NULL	Cytochrome P450 ( CYP ) epoxygenases	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochrome P450 ( CYP ) epoxygenases convert arachidonic acid to four epoxyeicosatrienoic acid ( EET ) regioisomers , 5 , 6 - , 8 , 9 - , 11 , 12 - , and 14 , 15-EET , that function as autacrine and paracrine mediators .
	manualset3
257159	2	425948	7	NULL	NULL	NULL	NULL	arachidonic acid 	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochrome P450 ( CYP ) epoxygenases convert arachidonic acid to four epoxyeicosatrienoic acid ( EET ) regioisomers , 5 , 6 - , 8 , 9 - , 11 , 12 - , and 14 , 15-EET , that function as autacrine and paracrine mediators .
	manualset3
257160	3	425948	7	NULL	NULL	NULL	NULL	four epoxyeicosatrienoic acid ( EET ) regioisomers	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochrome P450 ( CYP ) epoxygenases convert arachidonic acid to four epoxyeicosatrienoic acid ( EET ) regioisomers , 5 , 6 - , 8 , 9 - , 11 , 12 - , and 14 , 15-EET , that function as autacrine and paracrine mediators .
	manualset3
257161	4	425948	7	NULL	NULL	NULL	NULL	 5 , 6 - , 8 , 9 - , 11 , 12 -EET	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochrome P450 ( CYP ) epoxygenases convert arachidonic acid to four epoxyeicosatrienoic acid ( EET ) regioisomers , 5 , 6 - , 8 , 9 - , 11 , 12 - , and 14 , 15-EET , that function as autacrine and paracrine mediators .
	manualset3
257162	5	425948	7	NULL	NULL	NULL	NULL	14 , 15-EET	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochrome P450 ( CYP ) epoxygenases convert arachidonic acid to four epoxyeicosatrienoic acid ( EET ) regioisomers , 5 , 6 - , 8 , 9 - , 11 , 12 - , and 14 , 15-EET , that function as autacrine and paracrine mediators .
	manualset3
257163	6	425948	7	NULL	NULL	NULL	NULL	autacrine mediators	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochrome P450 ( CYP ) epoxygenases convert arachidonic acid to four epoxyeicosatrienoic acid ( EET ) regioisomers , 5 , 6 - , 8 , 9 - , 11 , 12 - , and 14 , 15-EET , that function as autacrine and paracrine mediators .
	manualset3
257164	7	425948	7	NULL	NULL	NULL	NULL	paracrine mediators	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochrome P450 ( CYP ) epoxygenases convert arachidonic acid to four epoxyeicosatrienoic acid ( EET ) regioisomers , 5 , 6 - , 8 , 9 - , 11 , 12 - , and 14 , 15-EET , that function as autacrine and paracrine mediators .
	manualset3
257165	1	425949	7	NULL	NULL	NULL	NULL	Cytochrome b561	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochrome b561 was inferred to function as the redox partner of the membrane-bound hydrogenase .
	manualset3
257166	2	425949	7	NULL	NULL	NULL	NULL	redox partner 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochrome b561 was inferred to function as the redox partner of the membrane-bound hydrogenase .
	manualset3
257167	3	425949	7	NULL	NULL	NULL	NULL	membrane-bound hydrogenase	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochrome b561 was inferred to function as the redox partner of the membrane-bound hydrogenase .
	manualset3
257168	1	425950	7	NULL	NULL	NULL	NULL	Microbial community	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Microbial community of freshwater sponges in Lake Bakal ) .
	manualset3
257169	2	425950	7	NULL	NULL	NULL	NULL	freshwater sponges 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Microbial community of freshwater sponges in Lake Bakal ) .
	manualset3
257170	3	425950	7	NULL	NULL	NULL	NULL	Lake Bakal	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Microbial community of freshwater sponges in Lake Bakal ) .
	manualset3
257171	1	425951	7	NULL	NULL	NULL	NULL	Cytochrome c oxidase ( EC 1.9.3.1 ) activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochrome c oxidase ( EC 1.9.3.1 ) activity of brown adipose tissue indicated a high rate of thermogenic activity in this tissue in LP rats , but ER animals showed some evidence of below normal function .
	manualset3
257172	2	425951	7	NULL	NULL	NULL	NULL	brown adipose tissue	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochrome c oxidase ( EC 1.9.3.1 ) activity of brown adipose tissue indicated a high rate of thermogenic activity in this tissue in LP rats , but ER animals showed some evidence of below normal function .
	manualset3
257173	3	425951	7	NULL	NULL	NULL	NULL	high rate	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochrome c oxidase ( EC 1.9.3.1 ) activity of brown adipose tissue indicated a high rate of thermogenic activity in this tissue in LP rats , but ER animals showed some evidence of below normal function .
	manualset3
257174	4	425951	7	NULL	NULL	NULL	NULL	 thermogenic activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochrome c oxidase ( EC 1.9.3.1 ) activity of brown adipose tissue indicated a high rate of thermogenic activity in this tissue in LP rats , but ER animals showed some evidence of below normal function .
	manualset3
257175	5	425951	7	NULL	NULL	NULL	NULL	tissue	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochrome c oxidase ( EC 1.9.3.1 ) activity of brown adipose tissue indicated a high rate of thermogenic activity in this tissue in LP rats , but ER animals showed some evidence of below normal function .
	manualset3
257176	6	425951	7	NULL	NULL	NULL	NULL	LP rats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochrome c oxidase ( EC 1.9.3.1 ) activity of brown adipose tissue indicated a high rate of thermogenic activity in this tissue in LP rats , but ER animals showed some evidence of below normal function .
	manualset3
257177	7	425951	7	NULL	NULL	NULL	NULL	ER animals	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochrome c oxidase ( EC 1.9.3.1 ) activity of brown adipose tissue indicated a high rate of thermogenic activity in this tissue in LP rats , but ER animals showed some evidence of below normal function .
	manualset3
257178	8	425951	7	NULL	NULL	NULL	NULL	evidence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochrome c oxidase ( EC 1.9.3.1 ) activity of brown adipose tissue indicated a high rate of thermogenic activity in this tissue in LP rats , but ER animals showed some evidence of below normal function .
	manualset3
257179	9	425951	7	NULL	NULL	NULL	NULL	normal function	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytochrome c oxidase ( EC 1.9.3.1 ) activity of brown adipose tissue indicated a high rate of thermogenic activity in this tissue in LP rats , but ER animals showed some evidence of below normal function .
	manualset3
257180	1	425952	7	NULL	NULL	NULL	NULL	Cytogenetic analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytogenetic analysis with GTG banding was performed on 1 , 000 lymphocyte metaphases per donor to identify genomic instability , including numerical and structural chromosomal aberrations , at a resolution of 10 Mb across the entire genome .
	manualset3
257181	2	425952	7	NULL	NULL	NULL	NULL	GTG banding	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytogenetic analysis with GTG banding was performed on 1 , 000 lymphocyte metaphases per donor to identify genomic instability , including numerical and structural chromosomal aberrations , at a resolution of 10 Mb across the entire genome .
	manualset3
257182	3	425952	7	NULL	NULL	NULL	NULL	1 , 000 lymphocyte metaphases per donor	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytogenetic analysis with GTG banding was performed on 1 , 000 lymphocyte metaphases per donor to identify genomic instability , including numerical and structural chromosomal aberrations , at a resolution of 10 Mb across the entire genome .
	manualset3
257183	4	425952	7	NULL	NULL	NULL	NULL	genomic instability	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytogenetic analysis with GTG banding was performed on 1 , 000 lymphocyte metaphases per donor to identify genomic instability , including numerical and structural chromosomal aberrations , at a resolution of 10 Mb across the entire genome .
	manualset3
257184	5	425952	7	NULL	NULL	NULL	NULL	numerical chromosomal aberrations	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytogenetic analysis with GTG banding was performed on 1 , 000 lymphocyte metaphases per donor to identify genomic instability , including numerical and structural chromosomal aberrations , at a resolution of 10 Mb across the entire genome .
	manualset3
257185	6	425952	7	NULL	NULL	NULL	NULL	structural chromosomal aberrations	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytogenetic analysis with GTG banding was performed on 1 , 000 lymphocyte metaphases per donor to identify genomic instability , including numerical and structural chromosomal aberrations , at a resolution of 10 Mb across the entire genome .
	manualset3
257186	7	425952	7	NULL	NULL	NULL	NULL	 resolution	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytogenetic analysis with GTG banding was performed on 1 , 000 lymphocyte metaphases per donor to identify genomic instability , including numerical and structural chromosomal aberrations , at a resolution of 10 Mb across the entire genome .
	manualset3
257187	8	425952	7	NULL	NULL	NULL	NULL	10 Mb	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytogenetic analysis with GTG banding was performed on 1 , 000 lymphocyte metaphases per donor to identify genomic instability , including numerical and structural chromosomal aberrations , at a resolution of 10 Mb across the entire genome .
	manualset3
257188	9	425952	7	NULL	NULL	NULL	NULL	 entire genome	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytogenetic analysis with GTG banding was performed on 1 , 000 lymphocyte metaphases per donor to identify genomic instability , including numerical and structural chromosomal aberrations , at a resolution of 10 Mb across the entire genome .
	manualset3
257189	1	425953	7	NULL	NULL	NULL	NULL	Cytogenetic studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytogenetic studies on human breast carcinomas .
	manualset3
257190	2	425953	7	NULL	NULL	NULL	NULL	 human breast carcinomas	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytogenetic studies on human breast carcinomas .
	manualset3
257191	1	425954	7	NULL	NULL	NULL	NULL	Cytokine determinants	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytokine determinants of viral tropism .
	manualset3
257192	2	425954	7	NULL	NULL	NULL	NULL	 viral tropism	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytokine determinants of viral tropism .
	manualset3
257193	1	425955	7	NULL	NULL	NULL	NULL	Cytokinesis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytokinesis : a comparative study of cytoplasmic division in animal cells .
	manualset3
257194	2	425955	7	NULL	NULL	NULL	NULL	comparative study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytokinesis : a comparative study of cytoplasmic division in animal cells .
	manualset3
257195	3	425955	7	NULL	NULL	NULL	NULL	 cytoplasmic division	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytokinesis : a comparative study of cytoplasmic division in animal cells .
	manualset3
257196	4	425955	7	NULL	NULL	NULL	NULL	animal cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytokinesis : a comparative study of cytoplasmic division in animal cells .
	manualset3
257197	1	425956	7	NULL	NULL	NULL	NULL	Cytokinesis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytokinesis during early development of a teleost embryo : Brachydanio rerio .
	manualset3
257198	2	425956	7	NULL	NULL	NULL	NULL	early development	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytokinesis during early development of a teleost embryo : Brachydanio rerio .
	manualset3
257199	3	425956	7	NULL	NULL	NULL	NULL	teleost embryo	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytokinesis during early development of a teleost embryo : Brachydanio rerio .
	manualset3
257200	4	425956	7	NULL	NULL	NULL	NULL	Brachydanio rerio	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytokinesis during early development of a teleost embryo : Brachydanio rerio .
	manualset3
257201	1	425957	7	NULL	NULL	NULL	NULL	Microbial flora	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Microbial flora of ulcer and its significance in the surgical treatment of the ulcer of the stomach and duodenum ) .
	manualset3
257202	2	425957	7	NULL	NULL	NULL	NULL	 ulcer	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Microbial flora of ulcer and its significance in the surgical treatment of the ulcer of the stomach and duodenum ) .
	manualset3
257203	3	425957	7	NULL	NULL	NULL	NULL	significance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Microbial flora of ulcer and its significance in the surgical treatment of the ulcer of the stomach and duodenum ) .
	manualset3
257204	4	425957	7	NULL	NULL	NULL	NULL	surgical treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Microbial flora of ulcer and its significance in the surgical treatment of the ulcer of the stomach and duodenum ) .
	manualset3
257205	5	425957	7	NULL	NULL	NULL	NULL	ulcer 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Microbial flora of ulcer and its significance in the surgical treatment of the ulcer of the stomach and duodenum ) .
	manualset3
257206	6	425957	7	NULL	NULL	NULL	NULL	stomach 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Microbial flora of ulcer and its significance in the surgical treatment of the ulcer of the stomach and duodenum ) .
	manualset3
257207	7	425957	7	NULL	NULL	NULL	NULL	duodenum 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Microbial flora of ulcer and its significance in the surgical treatment of the ulcer of the stomach and duodenum ) .
	manualset3
257208	1	425958	7	NULL	NULL	NULL	NULL	Cytology	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytology is a simple , rapid , and cost-effective means of examining PF , and can therefore play a significant role in establishing the diagnosis of BP .
	manualset3
257209	2	425958	7	NULL	NULL	NULL	NULL	 PF	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytology is a simple , rapid , and cost-effective means of examining PF , and can therefore play a significant role in establishing the diagnosis of BP .
	manualset3
257210	3	425958	7	NULL	NULL	NULL	NULL	role	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytology is a simple , rapid , and cost-effective means of examining PF , and can therefore play a significant role in establishing the diagnosis of BP .
	manualset3
257211	4	425958	7	NULL	NULL	NULL	NULL	diagnosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytology is a simple , rapid , and cost-effective means of examining PF , and can therefore play a significant role in establishing the diagnosis of BP .
	manualset3
257212	5	425958	7	NULL	NULL	NULL	NULL	BP	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytology is a simple , rapid , and cost-effective means of examining PF , and can therefore play a significant role in establishing the diagnosis of BP .
	manualset3
257213	1	425959	7	NULL	NULL	NULL	NULL	Cytolysis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytolysis by cloned helper T cells : induction by specific antigen or by anti-CD3 hybrid antibodies .
	manualset3
257214	2	425959	7	NULL	NULL	NULL	NULL	cloned helper T cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytolysis by cloned helper T cells : induction by specific antigen or by anti-CD3 hybrid antibodies .
	manualset3
257215	3	425959	7	NULL	NULL	NULL	NULL	 induction	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytolysis by cloned helper T cells : induction by specific antigen or by anti-CD3 hybrid antibodies .
	manualset3
257216	4	425959	7	NULL	NULL	NULL	NULL	specific antigen	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytolysis by cloned helper T cells : induction by specific antigen or by anti-CD3 hybrid antibodies .
	manualset3
257217	5	425959	7	NULL	NULL	NULL	NULL	anti-CD3 hybrid antibodies 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytolysis by cloned helper T cells : induction by specific antigen or by anti-CD3 hybrid antibodies .
	manualset3
257218	1	425960	7	NULL	NULL	NULL	NULL	Cytomorphological criteria	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytomorphological criteria , subclassifications of endocervical glandular cell abnormalities , and histopathological outcome : a frequency study .
	manualset3
257219	2	425960	7	NULL	NULL	NULL	NULL	subclassifications	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytomorphological criteria , subclassifications of endocervical glandular cell abnormalities , and histopathological outcome : a frequency study .
	manualset3
257220	3	425960	7	NULL	NULL	NULL	NULL	endocervical glandular cell abnormalities	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytomorphological criteria , subclassifications of endocervical glandular cell abnormalities , and histopathological outcome : a frequency study .
	manualset3
257221	4	425960	7	NULL	NULL	NULL	NULL	histopathological outcome	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytomorphological criteria , subclassifications of endocervical glandular cell abnormalities , and histopathological outcome : a frequency study .
	manualset3
257222	5	425960	7	NULL	NULL	NULL	NULL	frequency study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytomorphological criteria , subclassifications of endocervical glandular cell abnormalities , and histopathological outcome : a frequency study .
	manualset3
257223	1	425961	7	NULL	NULL	NULL	NULL	Cytoplasmic calcification	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytoplasmic calcification was seen in membrane-bound vesicles and as partially membrane-bound clusters of crystals .
	manualset3
257224	2	425961	7	NULL	NULL	NULL	NULL	membrane-bound vesicles	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytoplasmic calcification was seen in membrane-bound vesicles and as partially membrane-bound clusters of crystals .
	manualset3
257225	3	425961	7	NULL	NULL	NULL	NULL	membrane-bound clusters	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytoplasmic calcification was seen in membrane-bound vesicles and as partially membrane-bound clusters of crystals .
	manualset3
257226	4	425961	7	NULL	NULL	NULL	NULL	crystals	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytoplasmic calcification was seen in membrane-bound vesicles and as partially membrane-bound clusters of crystals .
	manualset3
257227	1	425962	7	NULL	NULL	NULL	NULL	Cytoplasmic inclusions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytoplasmic inclusions induced by wheat streak mosaic virus .
	manualset3
257228	2	425962	7	NULL	NULL	NULL	NULL	wheat streak mosaic virus	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytoplasmic inclusions induced by wheat streak mosaic virus .
	manualset3
257229	1	425963	7	NULL	NULL	NULL	NULL	Cytosine methylation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytosine methylation at promoter regions and late replication timing have both been implicated in the regulation of genes subject to X chromosome inactivation .
	manualset3
257230	2	425963	7	NULL	NULL	NULL	NULL	 promoter regions	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytosine methylation at promoter regions and late replication timing have both been implicated in the regulation of genes subject to X chromosome inactivation .
	manualset3
257231	3	425963	7	NULL	NULL	NULL	NULL	late replication timing	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytosine methylation at promoter regions and late replication timing have both been implicated in the regulation of genes subject to X chromosome inactivation .
	manualset3
257232	4	425963	7	NULL	NULL	NULL	NULL	regulation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytosine methylation at promoter regions and late replication timing have both been implicated in the regulation of genes subject to X chromosome inactivation .
	manualset3
257233	5	425963	7	NULL	NULL	NULL	NULL	genes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytosine methylation at promoter regions and late replication timing have both been implicated in the regulation of genes subject to X chromosome inactivation .
	manualset3
257234	6	425963	7	NULL	NULL	NULL	NULL	X chromosome inactivation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytosine methylation at promoter regions and late replication timing have both been implicated in the regulation of genes subject to X chromosome inactivation .
	manualset3
257235	1	425964	7	NULL	NULL	NULL	NULL	Cytosolic Ca2 + concentrations ( ( Ca2 + ) cyt )	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytosolic Ca2 + concentrations ( ( Ca2 + ) cyt ) and ( 3H ) inositol phosphates ( ( 3H ) InsP ) were correlated while varying the Ca2 + content of the sarcoplasmic reticulum ( SR ) in cultured A7r5 cells at rest and during activation with ( Arg8 ) - vasopressin ( AVP ) .
	manualset3
257236	2	425964	7	NULL	NULL	NULL	NULL	( 3H ) inositol phosphates ( ( 3H ) InsP ) 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytosolic Ca2 + concentrations ( ( Ca2 + ) cyt ) and ( 3H ) inositol phosphates ( ( 3H ) InsP ) were correlated while varying the Ca2 + content of the sarcoplasmic reticulum ( SR ) in cultured A7r5 cells at rest and during activation with ( Arg8 ) - vasopressin ( AVP ) .
	manualset3
257237	3	425964	7	NULL	NULL	NULL	NULL	Ca2 + content	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytosolic Ca2 + concentrations ( ( Ca2 + ) cyt ) and ( 3H ) inositol phosphates ( ( 3H ) InsP ) were correlated while varying the Ca2 + content of the sarcoplasmic reticulum ( SR ) in cultured A7r5 cells at rest and during activation with ( Arg8 ) - vasopressin ( AVP ) .
	manualset3
257238	4	425964	7	NULL	NULL	NULL	NULL	sarcoplasmic reticulum ( SR )	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytosolic Ca2 + concentrations ( ( Ca2 + ) cyt ) and ( 3H ) inositol phosphates ( ( 3H ) InsP ) were correlated while varying the Ca2 + content of the sarcoplasmic reticulum ( SR ) in cultured A7r5 cells at rest and during activation with ( Arg8 ) - vasopressin ( AVP ) .
	manualset3
257239	5	425964	7	NULL	NULL	NULL	NULL	cultured A7r5 cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytosolic Ca2 + concentrations ( ( Ca2 + ) cyt ) and ( 3H ) inositol phosphates ( ( 3H ) InsP ) were correlated while varying the Ca2 + content of the sarcoplasmic reticulum ( SR ) in cultured A7r5 cells at rest and during activation with ( Arg8 ) - vasopressin ( AVP ) .
	manualset3
257240	6	425964	7	NULL	NULL	NULL	NULL	activation 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytosolic Ca2 + concentrations ( ( Ca2 + ) cyt ) and ( 3H ) inositol phosphates ( ( 3H ) InsP ) were correlated while varying the Ca2 + content of the sarcoplasmic reticulum ( SR ) in cultured A7r5 cells at rest and during activation with ( Arg8 ) - vasopressin ( AVP ) .
	manualset3
257241	7	425964	7	NULL	NULL	NULL	NULL	( Arg8 ) - vasopressin ( AVP )	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytosolic Ca2 + concentrations ( ( Ca2 + ) cyt ) and ( 3H ) inositol phosphates ( ( 3H ) InsP ) were correlated while varying the Ca2 + content of the sarcoplasmic reticulum ( SR ) in cultured A7r5 cells at rest and during activation with ( Arg8 ) - vasopressin ( AVP ) .
	manualset3
257242	1	425965	7	NULL	NULL	NULL	NULL	Cytosolic Ca2 +	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytosolic Ca2 + increases in response to K ( + ) - induced depolarization of the cardiomyocytes were much less sensitive to cocaine than the electrically induced Ca2 + transients .
	manualset3
257243	2	425965	7	NULL	NULL	NULL	NULL	 K ( + ) - induced depolarization	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytosolic Ca2 + increases in response to K ( + ) - induced depolarization of the cardiomyocytes were much less sensitive to cocaine than the electrically induced Ca2 + transients .
	manualset3
257244	3	425965	7	NULL	NULL	NULL	NULL	cardiomyocytes	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytosolic Ca2 + increases in response to K ( + ) - induced depolarization of the cardiomyocytes were much less sensitive to cocaine than the electrically induced Ca2 + transients .
	manualset3
257245	4	425965	7	NULL	NULL	NULL	NULL	cocaine	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytosolic Ca2 + increases in response to K ( + ) - induced depolarization of the cardiomyocytes were much less sensitive to cocaine than the electrically induced Ca2 + transients .
	manualset3
257246	5	425965	7	NULL	NULL	NULL	NULL	electrically induced Ca2 + transients	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytosolic Ca2 + increases in response to K ( + ) - induced depolarization of the cardiomyocytes were much less sensitive to cocaine than the electrically induced Ca2 + transients .
	manualset3
257247	1	425966	7	NULL	NULL	NULL	NULL	Cytosolic NADPH	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytosolic NADPH is the electron donor for extracellular fe reduction in iron-deficient bean roots .
	manualset3
257248	2	425966	7	NULL	NULL	NULL	NULL	electron donor	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytosolic NADPH is the electron donor for extracellular fe reduction in iron-deficient bean roots .
	manualset3
257249	3	425966	7	NULL	NULL	NULL	NULL	extracellular fe reduction	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytosolic NADPH is the electron donor for extracellular fe reduction in iron-deficient bean roots .
	manualset3
257250	4	425966	7	NULL	NULL	NULL	NULL	iron-deficient bean roots	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytosolic NADPH is the electron donor for extracellular fe reduction in iron-deficient bean roots .
	manualset3
257251	1	425967	7	NULL	NULL	NULL	NULL	Cytosolic concentrations	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytosolic concentrations and transmembrane fluxes of NH4 + / NH3 .
	manualset3
257252	2	425967	7	NULL	NULL	NULL	NULL	transmembrane fluxes	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytosolic concentrations and transmembrane fluxes of NH4 + / NH3 .
	manualset3
257253	3	425967	7	NULL	NULL	NULL	NULL	NH4 + / NH3	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytosolic concentrations and transmembrane fluxes of NH4 + / NH3 .
	manualset3
257254	1	425968	7	NULL	NULL	NULL	NULL	Microbiological control	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Microbiological control of solutions for internal administration ) .
	manualset3
257255	2	425968	7	NULL	NULL	NULL	NULL	solutions	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Microbiological control of solutions for internal administration ) .
	manualset3
257256	3	425968	7	NULL	NULL	NULL	NULL	internal administration	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Microbiological control of solutions for internal administration ) .
	manualset3
257258	1	425969	7	NULL	NULL	NULL	NULL	Cytosolic free Ca ( 2 + ) mobilization 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytosolic free Ca ( 2 + ) mobilization induced by microbe/pathogen-associated molecular patterns ( MAMPs/PAMPs ) play key roles in plant innate immunity .
	manualset3
257261	2	425969	7	NULL	NULL	NULL	NULL	microbe/pathogen-associated molecular patterns ( MAMPs/PAMPs )	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytosolic free Ca ( 2 + ) mobilization induced by microbe/pathogen-associated molecular patterns ( MAMPs/PAMPs ) play key roles in plant innate immunity .
	manualset3
257262	3	425969	7	NULL	NULL	NULL	NULL	key roles	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytosolic free Ca ( 2 + ) mobilization induced by microbe/pathogen-associated molecular patterns ( MAMPs/PAMPs ) play key roles in plant innate immunity .
	manualset3
257263	4	425969	7	NULL	NULL	NULL	NULL	plant innate immunity 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytosolic free Ca ( 2 + ) mobilization induced by microbe/pathogen-associated molecular patterns ( MAMPs/PAMPs ) play key roles in plant innate immunity .
	manualset3
257264	1	425970	7	NULL	NULL	NULL	NULL	Cytotoxic activity 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytotoxic activity of Staphylococcus hyicus .
	manualset3
257265	2	425970	7	NULL	NULL	NULL	NULL	Staphylococcus hyicus	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytotoxic activity of Staphylococcus hyicus .
	manualset3
257268	1	425971	7	NULL	NULL	NULL	NULL	Cytotoxic effect 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytotoxic effect of prolamin-derived peptides on in vitro cultures of cell line Caco-2 : Implications for coeliac disease .
	manualset3
257269	2	425971	7	NULL	NULL	NULL	NULL	prolamin-derived peptides	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytotoxic effect of prolamin-derived peptides on in vitro cultures of cell line Caco-2 : Implications for coeliac disease .
	manualset3
257270	3	425971	7	NULL	NULL	NULL	NULL	in vitro cultures	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytotoxic effect of prolamin-derived peptides on in vitro cultures of cell line Caco-2 : Implications for coeliac disease .
	manualset3
257272	4	425971	7	NULL	NULL	NULL	NULL	cell line Caco-2	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytotoxic effect of prolamin-derived peptides on in vitro cultures of cell line Caco-2 : Implications for coeliac disease .
	manualset3
257273	5	425971	7	NULL	NULL	NULL	NULL	Implications	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytotoxic effect of prolamin-derived peptides on in vitro cultures of cell line Caco-2 : Implications for coeliac disease .
	manualset3
257274	6	425971	7	NULL	NULL	NULL	NULL	coeliac disease 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytotoxic effect of prolamin-derived peptides on in vitro cultures of cell line Caco-2 : Implications for coeliac disease .
	manualset3
257580	1	425972	7	NULL	NULL	NULL	NULL	Cytotoxicity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytotoxicity by 24-h exposure of hNAT - or hOCT-expressing cells to low DSP4 concentrations ( & lt ; 10 microM ) could be observed only in hNAT-expressing cells .
	manualset3
257581	2	425972	7	NULL	NULL	NULL	NULL	 24-h exposure	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytotoxicity by 24-h exposure of hNAT - or hOCT-expressing cells to low DSP4 concentrations ( & lt ; 10 microM ) could be observed only in hNAT-expressing cells .
	manualset3
257582	3	425972	7	NULL	NULL	NULL	NULL	hNAT - expressing cells 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytotoxicity by 24-h exposure of hNAT - or hOCT-expressing cells to low DSP4 concentrations ( & lt ; 10 microM ) could be observed only in hNAT-expressing cells .
	manualset3
257583	4	425972	7	NULL	NULL	NULL	NULL	hOCT-expressing cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytotoxicity by 24-h exposure of hNAT - or hOCT-expressing cells to low DSP4 concentrations ( & lt ; 10 microM ) could be observed only in hNAT-expressing cells .
	manualset3
257584	5	425972	7	NULL	NULL	NULL	NULL	 low DSP4 concentrations 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytotoxicity by 24-h exposure of hNAT - or hOCT-expressing cells to low DSP4 concentrations ( & lt ; 10 microM ) could be observed only in hNAT-expressing cells .
	manualset3
257585	6	425972	7	NULL	NULL	NULL	NULL	& lt ; 10 microM	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytotoxicity by 24-h exposure of hNAT - or hOCT-expressing cells to low DSP4 concentrations ( & lt ; 10 microM ) could be observed only in hNAT-expressing cells .
	manualset3
257586	7	425972	7	NULL	NULL	NULL	NULL	hNAT-expressing cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytotoxicity by 24-h exposure of hNAT - or hOCT-expressing cells to low DSP4 concentrations ( & lt ; 10 microM ) could be observed only in hNAT-expressing cells .
	manualset3
257587	1	425973	7	NULL	NULL	NULL	NULL	Cytotype IV	Chromosome												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytotype IV presented CMA ( 3 ) and DAPI positive heterochromatin .
	manualset3
257588	2	425973	7	NULL	NULL	NULL	NULL	CMA ( 3 ) 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytotype IV presented CMA ( 3 ) and DAPI positive heterochromatin .
	manualset3
257589	3	425973	7	NULL	NULL	NULL	NULL	DAPI positive heterochromatin	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Cytotype IV presented CMA ( 3 ) and DAPI positive heterochromatin .
	manualset3
257594	1	425974	7	NULL	NULL	NULL	NULL	D-2 ( controlled-release MK-458 )	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	D-2 ( controlled-release MK-458 ) vs combined D-1 and D-2 ( pergolide )
	manualset3
257595	2	425974	7	NULL	NULL	NULL	NULL	combined D-1 pergolide 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	D-2 ( controlled-release MK-458 ) vs combined D-1 and D-2 ( pergolide )
	manualset3
257596	3	425974	7	NULL	NULL	NULL	NULL	 D-2 ( pergolide )	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	D-2 ( controlled-release MK-458 ) vs combined D-1 and D-2 ( pergolide )
	manualset3
257597	1	425975	7	NULL	NULL	NULL	NULL	D-Amphetamine 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	D-Amphetamine ( 0.1-5 microM ) , as well as dopamine , produced a dose-dependent decrease of the excitatory synaptic potentials .
	manualset3
257598	2	425975	7	NULL	NULL	NULL	NULL	0.1-5 microM	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	D-Amphetamine ( 0.1-5 microM ) , as well as dopamine , produced a dose-dependent decrease of the excitatory synaptic potentials .
	manualset3
257600	3	425975	7	NULL	NULL	NULL	NULL	 dopamine 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	D-Amphetamine ( 0.1-5 microM ) , as well as dopamine , produced a dose-dependent decrease of the excitatory synaptic potentials .
	manualset3
257601	4	425975	7	NULL	NULL	NULL	NULL	dose-dependent decrease	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	D-Amphetamine ( 0.1-5 microM ) , as well as dopamine , produced a dose-dependent decrease of the excitatory synaptic potentials .
	manualset3
257602	5	425975	7	NULL	NULL	NULL	NULL	 excitatory synaptic potentials	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	D-Amphetamine ( 0.1-5 microM ) , as well as dopamine , produced a dose-dependent decrease of the excitatory synaptic potentials .
	manualset3
257625	1	425976	7	NULL	NULL	NULL	NULL	Micromorphology	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Micromorphology of the nephgon in its relation to function .
	manualset3
257626	2	425976	7	NULL	NULL	NULL	NULL	nephgon 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Micromorphology of the nephgon in its relation to function .
	manualset3
257627	3	425976	7	NULL	NULL	NULL	NULL	relation	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Micromorphology of the nephgon in its relation to function .
	manualset3
257628	4	425976	7	NULL	NULL	NULL	NULL	function	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Micromorphology of the nephgon in its relation to function .
	manualset3
257629	1	425977	7	NULL	NULL	NULL	NULL	D-Phe2 , 6	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	D-Phe2 , 6 , Pro3-GnRH was not able to initiate courtship behavior during the nonbreeding season , indicating that courtship behavior is dependent on the interaction of multiple components .
	manualset3
257630	2	425977	7	NULL	NULL	NULL	NULL	Pro3-GnRH	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	D-Phe2 , 6 , Pro3-GnRH was not able to initiate courtship behavior during the nonbreeding season , indicating that courtship behavior is dependent on the interaction of multiple components .
	manualset3
257631	3	425977	7	NULL	NULL	NULL	NULL	 courtship behavior 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	D-Phe2 , 6 , Pro3-GnRH was not able to initiate courtship behavior during the nonbreeding season , indicating that courtship behavior is dependent on the interaction of multiple components .
	manualset3
257632	4	425977	7	NULL	NULL	NULL	NULL	nonbreeding season 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	D-Phe2 , 6 , Pro3-GnRH was not able to initiate courtship behavior during the nonbreeding season , indicating that courtship behavior is dependent on the interaction of multiple components .
	manualset3
257633	5	425977	7	NULL	NULL	NULL	NULL	courtship behavior	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	D-Phe2 , 6 , Pro3-GnRH was not able to initiate courtship behavior during the nonbreeding season , indicating that courtship behavior is dependent on the interaction of multiple components .
	manualset3
257634	6	425977	7	NULL	NULL	NULL	NULL	 interaction	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	D-Phe2 , 6 , Pro3-GnRH was not able to initiate courtship behavior during the nonbreeding season , indicating that courtship behavior is dependent on the interaction of multiple components .
	manualset3
257635	7	425977	7	NULL	NULL	NULL	NULL	multiple components	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	D-Phe2 , 6 , Pro3-GnRH was not able to initiate courtship behavior during the nonbreeding season , indicating that courtship behavior is dependent on the interaction of multiple components .
	manualset3
257636	1	425978	7	NULL	NULL	NULL	NULL	D ( - ) - beta-hydroxybutyrate dehydrogenase activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	D ( - ) - beta-hydroxybutyrate dehydrogenase activity in cloned cell lines of glial and neuronal origin .
	manualset3
257637	2	425978	7	NULL	NULL	NULL	NULL	cloned cell lines 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	D ( - ) - beta-hydroxybutyrate dehydrogenase activity in cloned cell lines of glial and neuronal origin .
	manualset3
257638	3	425978	7	NULL	NULL	NULL	NULL	glial origin	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	D ( - ) - beta-hydroxybutyrate dehydrogenase activity in cloned cell lines of glial and neuronal origin .
	manualset3
257639	4	425978	7	NULL	NULL	NULL	NULL	neuronal origin	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	D ( - ) - beta-hydroxybutyrate dehydrogenase activity in cloned cell lines of glial and neuronal origin .
	manualset3
257640	1	425979	7	NULL	NULL	NULL	NULL	D2E7	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	D2E7 has a higher affinity for TNFalpha than 2SD4 and the two antibodies ( Abs ) differ by 12 amino acids in the antigen ( Ag ) binding regions .
	manualset3
257641	2	425979	7	NULL	NULL	NULL	NULL	higher affinity 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	D2E7 has a higher affinity for TNFalpha than 2SD4 and the two antibodies ( Abs ) differ by 12 amino acids in the antigen ( Ag ) binding regions .
	manualset3
257642	3	425979	7	NULL	NULL	NULL	NULL	TNFalpha	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	D2E7 has a higher affinity for TNFalpha than 2SD4 and the two antibodies ( Abs ) differ by 12 amino acids in the antigen ( Ag ) binding regions .
	manualset3
257643	4	425979	7	NULL	NULL	NULL	NULL	2SD4	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	D2E7 has a higher affinity for TNFalpha than 2SD4 and the two antibodies ( Abs ) differ by 12 amino acids in the antigen ( Ag ) binding regions .
	manualset3
257645	5	425979	7	NULL	NULL	NULL	NULL	 two antibodies ( Abs )	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	D2E7 has a higher affinity for TNFalpha than 2SD4 and the two antibodies ( Abs ) differ by 12 amino acids in the antigen ( Ag ) binding regions .
	manualset3
257646	6	425979	7	NULL	NULL	NULL	NULL	12 amino acids	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	D2E7 has a higher affinity for TNFalpha than 2SD4 and the two antibodies ( Abs ) differ by 12 amino acids in the antigen ( Ag ) binding regions .
	manualset3
257647	7	425979	7	NULL	NULL	NULL	NULL	antigen ( Ag ) binding regions	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	D2E7 has a higher affinity for TNFalpha than 2SD4 and the two antibodies ( Abs ) differ by 12 amino acids in the antigen ( Ag ) binding regions .
	manualset3
257648	1	425980	7	NULL	NULL	NULL	NULL	DAG	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DAG , a product of phospholipase C ( PLC ) - catalyzed breakdown of phosphoinositides , stimulates protein kinase C. Ca2 + ionophores and phorbol esters ( or DAG analogs ) elicit a synergistic secretory response in the exocrine pancreas and parotid gland .
	manualset3
257649	2	425980	7	NULL	NULL	NULL	NULL	 product 	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DAG , a product of phospholipase C ( PLC ) - catalyzed breakdown of phosphoinositides , stimulates protein kinase C. Ca2 + ionophores and phorbol esters ( or DAG analogs ) elicit a synergistic secretory response in the exocrine pancreas and parotid gland .
	manualset3
257650	3	425980	7	NULL	NULL	NULL	NULL	phospholipase C ( PLC ) - catalyzed breakdown	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DAG , a product of phospholipase C ( PLC ) - catalyzed breakdown of phosphoinositides , stimulates protein kinase C. Ca2 + ionophores and phorbol esters ( or DAG analogs ) elicit a synergistic secretory response in the exocrine pancreas and parotid gland .
	manualset3
257652	4	425980	7	NULL	NULL	NULL	NULL	phosphoinositides	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DAG , a product of phospholipase C ( PLC ) - catalyzed breakdown of phosphoinositides , stimulates protein kinase C. Ca2 + ionophores and phorbol esters ( or DAG analogs ) elicit a synergistic secretory response in the exocrine pancreas and parotid gland .
	manualset3
257654	5	425980	7	NULL	NULL	NULL	NULL	 protein kinase C	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DAG , a product of phospholipase C ( PLC ) - catalyzed breakdown of phosphoinositides , stimulates protein kinase C. Ca2 + ionophores and phorbol esters ( or DAG analogs ) elicit a synergistic secretory response in the exocrine pancreas and parotid gland .
	manualset3
257655	6	425980	7	NULL	NULL	NULL	NULL	Ca2 + ionophores	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DAG , a product of phospholipase C ( PLC ) - catalyzed breakdown of phosphoinositides , stimulates protein kinase C. Ca2 + ionophores and phorbol esters ( or DAG analogs ) elicit a synergistic secretory response in the exocrine pancreas and parotid gland .
	manualset3
257656	7	425980	7	NULL	NULL	NULL	NULL	phorbol esters 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DAG , a product of phospholipase C ( PLC ) - catalyzed breakdown of phosphoinositides , stimulates protein kinase C. Ca2 + ionophores and phorbol esters ( or DAG analogs ) elicit a synergistic secretory response in the exocrine pancreas and parotid gland .
	manualset3
257657	8	425980	7	NULL	NULL	NULL	NULL	DAG analogs	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DAG , a product of phospholipase C ( PLC ) - catalyzed breakdown of phosphoinositides , stimulates protein kinase C. Ca2 + ionophores and phorbol esters ( or DAG analogs ) elicit a synergistic secretory response in the exocrine pancreas and parotid gland .
	manualset3
257659	9	425980	7	NULL	NULL	NULL	NULL	synergistic secretory response	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DAG , a product of phospholipase C ( PLC ) - catalyzed breakdown of phosphoinositides , stimulates protein kinase C. Ca2 + ionophores and phorbol esters ( or DAG analogs ) elicit a synergistic secretory response in the exocrine pancreas and parotid gland .
	manualset3
257660	10	425980	7	NULL	NULL	NULL	NULL	 exocrine pancreas	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DAG , a product of phospholipase C ( PLC ) - catalyzed breakdown of phosphoinositides , stimulates protein kinase C. Ca2 + ionophores and phorbol esters ( or DAG analogs ) elicit a synergistic secretory response in the exocrine pancreas and parotid gland .
	manualset3
257662	11	425980	7	NULL	NULL	NULL	NULL	parotid gland 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DAG , a product of phospholipase C ( PLC ) - catalyzed breakdown of phosphoinositides , stimulates protein kinase C. Ca2 + ionophores and phorbol esters ( or DAG analogs ) elicit a synergistic secretory response in the exocrine pancreas and parotid gland .
	manualset3
257757	1	425981	7	NULL	NULL	NULL	NULL	DCregs	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DCregs expressed significantly higher levels of CD45RB and produced significantly less IL-12 compared with conventional dendritic cells .
	manualset3
257758	2	425981	7	NULL	NULL	NULL	NULL	higher levels 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DCregs expressed significantly higher levels of CD45RB and produced significantly less IL-12 compared with conventional dendritic cells .
	manualset3
257759	3	425981	7	NULL	NULL	NULL	NULL	CD45RB	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DCregs expressed significantly higher levels of CD45RB and produced significantly less IL-12 compared with conventional dendritic cells .
	manualset3
257760	4	425981	7	NULL	NULL	NULL	NULL	IL-12	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DCregs expressed significantly higher levels of CD45RB and produced significantly less IL-12 compared with conventional dendritic cells .
	manualset3
257761	5	425981	7	NULL	NULL	NULL	NULL	dendritic cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DCregs expressed significantly higher levels of CD45RB and produced significantly less IL-12 compared with conventional dendritic cells .
	manualset3
257762	1	425982	7	NULL	NULL	NULL	NULL	DCs	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DCs treated with single TLR agonists induced IL-17A production by allogeneic and Ag-specific memory CD4 ( + ) T cells , an effect that was abrogated by IL-23 neutralization .
	manualset3
257763	2	425982	7	NULL	NULL	NULL	NULL	single TLR agonists	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DCs treated with single TLR agonists induced IL-17A production by allogeneic and Ag-specific memory CD4 ( + ) T cells , an effect that was abrogated by IL-23 neutralization .
	manualset3
257765	3	425982	7	NULL	NULL	NULL	NULL	IL-17A production	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DCs treated with single TLR agonists induced IL-17A production by allogeneic and Ag-specific memory CD4 ( + ) T cells , an effect that was abrogated by IL-23 neutralization .
	manualset3
257768	4	425982	7	NULL	NULL	NULL	NULL	allogeneic specific memory CD4 ( + ) T cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DCs treated with single TLR agonists induced IL-17A production by allogeneic and Ag-specific memory CD4 ( + ) T cells , an effect that was abrogated by IL-23 neutralization .
	manualset3
257770	5	425982	7	NULL	NULL	NULL	NULL	Ag-specific memory CD4 ( + ) T cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DCs treated with single TLR agonists induced IL-17A production by allogeneic and Ag-specific memory CD4 ( + ) T cells , an effect that was abrogated by IL-23 neutralization .
	manualset3
257771	7	425982	7	NULL	NULL	NULL	NULL	 IL-23 neutralization	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DCs treated with single TLR agonists induced IL-17A production by allogeneic and Ag-specific memory CD4 ( + ) T cells , an effect that was abrogated by IL-23 neutralization .
	manualset3
257774	6	425982	7	NULL	NULL	NULL	NULL	effect	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DCs treated with single TLR agonists induced IL-17A production by allogeneic and Ag-specific memory CD4 ( + ) T cells , an effect that was abrogated by IL-23 neutralization .
	manualset3
257778	1	425983	7	NULL	NULL	NULL	NULL	DEC	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DEC inhibited proliferation of these cells , and cells grown in the presence of DEC were likely to separate from each other and became round in shape .
	manualset3
257779	2	425983	7	NULL	NULL	NULL	NULL	proliferation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DEC inhibited proliferation of these cells , and cells grown in the presence of DEC were likely to separate from each other and became round in shape .
	manualset3
257780	3	425983	7	NULL	NULL	NULL	NULL	 cells 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DEC inhibited proliferation of these cells , and cells grown in the presence of DEC were likely to separate from each other and became round in shape .
	manualset3
257781	4	425983	7	NULL	NULL	NULL	NULL	 cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DEC inhibited proliferation of these cells , and cells grown in the presence of DEC were likely to separate from each other and became round in shape .
	manualset3
257782	5	425983	7	NULL	NULL	NULL	NULL	presence 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DEC inhibited proliferation of these cells , and cells grown in the presence of DEC were likely to separate from each other and became round in shape .
	manualset3
257783	6	425983	7	NULL	NULL	NULL	NULL	DEC	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DEC inhibited proliferation of these cells , and cells grown in the presence of DEC were likely to separate from each other and became round in shape .
	manualset3
257786	7	425983	7	NULL	NULL	NULL	NULL	 round	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DEC inhibited proliferation of these cells , and cells grown in the presence of DEC were likely to separate from each other and became round in shape .
	manualset3
257789	8	425983	7	NULL	NULL	NULL	NULL	 shape	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DEC inhibited proliferation of these cells , and cells grown in the presence of DEC were likely to separate from each other and became round in shape .
	manualset3
257791	1	425984	7	NULL	NULL	NULL	NULL	DEPRESSION	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DEPRESSION OF THE TUBERCULIN REACTION BY VIRAL VACCINES .
	manualset3
257792	2	425984	7	NULL	NULL	NULL	NULL	TUBERCULIN REACTION	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DEPRESSION OF THE TUBERCULIN REACTION BY VIRAL VACCINES .
	manualset3
257794	3	425984	7	NULL	NULL	NULL	NULL	VIRAL VACCINES	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DEPRESSION OF THE TUBERCULIN REACTION BY VIRAL VACCINES .
	manualset3
257803	1	425985	7	NULL	NULL	NULL	NULL	DES	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DES , IOX and propilthyouracil ( PTU , a goitrogen ) were administered in the diet to sea bream juveniles at 1 mg/kg fish ( n = 14/treatment ) for 21 days .
	manualset3
257804	2	425985	7	NULL	NULL	NULL	NULL	IOX 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DES , IOX and propilthyouracil ( PTU , a goitrogen ) were administered in the diet to sea bream juveniles at 1 mg/kg fish ( n = 14/treatment ) for 21 days .
	manualset3
257805	3	425985	7	NULL	NULL	NULL	NULL	propilthyouracil	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DES , IOX and propilthyouracil ( PTU , a goitrogen ) were administered in the diet to sea bream juveniles at 1 mg/kg fish ( n = 14/treatment ) for 21 days .
	manualset3
257806	4	425985	7	NULL	NULL	NULL	NULL	PTU	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DES , IOX and propilthyouracil ( PTU , a goitrogen ) were administered in the diet to sea bream juveniles at 1 mg/kg fish ( n = 14/treatment ) for 21 days .
	manualset3
257807	5	425985	7	NULL	NULL	NULL	NULL	goitrogen 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DES , IOX and propilthyouracil ( PTU , a goitrogen ) were administered in the diet to sea bream juveniles at 1 mg/kg fish ( n = 14/treatment ) for 21 days .
	manualset3
257808	6	425985	7	NULL	NULL	NULL	NULL	diet 	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DES , IOX and propilthyouracil ( PTU , a goitrogen ) were administered in the diet to sea bream juveniles at 1 mg/kg fish ( n = 14/treatment ) for 21 days .
	manualset3
257810	7	425985	7	NULL	NULL	NULL	NULL	sea bream juveniles	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DES , IOX and propilthyouracil ( PTU , a goitrogen ) were administered in the diet to sea bream juveniles at 1 mg/kg fish ( n = 14/treatment ) for 21 days .
	manualset3
257812	8	425985	7	NULL	NULL	NULL	NULL	1 mg/kg fish	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DES , IOX and propilthyouracil ( PTU , a goitrogen ) were administered in the diet to sea bream juveniles at 1 mg/kg fish ( n = 14/treatment ) for 21 days .
	manualset3
257814	9	425985	7	NULL	NULL	NULL	NULL	 n = 14/treatment	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DES , IOX and propilthyouracil ( PTU , a goitrogen ) were administered in the diet to sea bream juveniles at 1 mg/kg fish ( n = 14/treatment ) for 21 days .
	manualset3
257815	10	425985	7	NULL	NULL	NULL	NULL	21 days	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DES , IOX and propilthyouracil ( PTU , a goitrogen ) were administered in the diet to sea bream juveniles at 1 mg/kg fish ( n = 14/treatment ) for 21 days .
	manualset3
257817	1	425986	7	NULL	NULL	NULL	NULL	DEVELOPMENT	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DEVELOPMENT AND CONCLUSIONS : In spite of many studies confirming the importance of genetic factors in the occurrence of idiopathic epilepsy , these appear to be complex and probably involve a locus of variable expression or several loci with similar phenotype expression ( epistaxis ) .
	manualset3
257824	2	425986	7	NULL	NULL	NULL	NULL	 CONCLUSIONS	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DEVELOPMENT AND CONCLUSIONS : In spite of many studies confirming the importance of genetic factors in the occurrence of idiopathic epilepsy , these appear to be complex and probably involve a locus of variable expression or several loci with similar phenotype expression ( epistaxis ) .
	manualset3
257826	3	425986	7	NULL	NULL	NULL	NULL	 studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DEVELOPMENT AND CONCLUSIONS : In spite of many studies confirming the importance of genetic factors in the occurrence of idiopathic epilepsy , these appear to be complex and probably involve a locus of variable expression or several loci with similar phenotype expression ( epistaxis ) .
	manualset3
257827	4	425986	7	NULL	NULL	NULL	NULL	 genetic factors	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DEVELOPMENT AND CONCLUSIONS : In spite of many studies confirming the importance of genetic factors in the occurrence of idiopathic epilepsy , these appear to be complex and probably involve a locus of variable expression or several loci with similar phenotype expression ( epistaxis ) .
	manualset3
257828	5	425986	7	NULL	NULL	NULL	NULL	 occurrence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DEVELOPMENT AND CONCLUSIONS : In spite of many studies confirming the importance of genetic factors in the occurrence of idiopathic epilepsy , these appear to be complex and probably involve a locus of variable expression or several loci with similar phenotype expression ( epistaxis ) .
	manualset3
257829	6	425986	7	NULL	NULL	NULL	NULL	idiopathic epilepsy	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DEVELOPMENT AND CONCLUSIONS : In spite of many studies confirming the importance of genetic factors in the occurrence of idiopathic epilepsy , these appear to be complex and probably involve a locus of variable expression or several loci with similar phenotype expression ( epistaxis ) .
	manualset3
257832	7	425986	7	NULL	NULL	NULL	NULL	 locus	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DEVELOPMENT AND CONCLUSIONS : In spite of many studies confirming the importance of genetic factors in the occurrence of idiopathic epilepsy , these appear to be complex and probably involve a locus of variable expression or several loci with similar phenotype expression ( epistaxis ) .
	manualset3
257833	8	425986	7	NULL	NULL	NULL	NULL	variable expression 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DEVELOPMENT AND CONCLUSIONS : In spite of many studies confirming the importance of genetic factors in the occurrence of idiopathic epilepsy , these appear to be complex and probably involve a locus of variable expression or several loci with similar phenotype expression ( epistaxis ) .
	manualset3
257834	9	425986	7	NULL	NULL	NULL	NULL	loci	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DEVELOPMENT AND CONCLUSIONS : In spite of many studies confirming the importance of genetic factors in the occurrence of idiopathic epilepsy , these appear to be complex and probably involve a locus of variable expression or several loci with similar phenotype expression ( epistaxis ) .
	manualset3
257835	10	425986	7	NULL	NULL	NULL	NULL	phenotype expression 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DEVELOPMENT AND CONCLUSIONS : In spite of many studies confirming the importance of genetic factors in the occurrence of idiopathic epilepsy , these appear to be complex and probably involve a locus of variable expression or several loci with similar phenotype expression ( epistaxis ) .
	manualset3
257836	11	425986	7	NULL	NULL	NULL	NULL	epistaxis 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DEVELOPMENT AND CONCLUSIONS : In spite of many studies confirming the importance of genetic factors in the occurrence of idiopathic epilepsy , these appear to be complex and probably involve a locus of variable expression or several loci with similar phenotype expression ( epistaxis ) .
	manualset3
257840	1	425987	7	NULL	NULL	NULL	NULL	Microtubules 	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Microtubules : functional polymorphisms of tubulin and associated proteins ( structural and motor MAP 's ) ) .
	manualset3
257841	2	425987	7	NULL	NULL	NULL	NULL	 functional polymorphisms	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Microtubules : functional polymorphisms of tubulin and associated proteins ( structural and motor MAP 's ) ) .
	manualset3
257844	3	425987	7	NULL	NULL	NULL	NULL	 tubulin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Microtubules : functional polymorphisms of tubulin and associated proteins ( structural and motor MAP 's ) ) .
	manualset3
257845	4	425987	7	NULL	NULL	NULL	NULL	associated proteins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Microtubules : functional polymorphisms of tubulin and associated proteins ( structural and motor MAP 's ) ) .
	manualset3
257847	5	425987	7	NULL	NULL	NULL	NULL	 structural MAP's	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Microtubules : functional polymorphisms of tubulin and associated proteins ( structural and motor MAP 's ) ) .
	manualset3
257849	6	425987	7	NULL	NULL	NULL	NULL	 motor MAP 's	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Microtubules : functional polymorphisms of tubulin and associated proteins ( structural and motor MAP 's ) ) .
	manualset3
257853	1	425988	7	NULL	NULL	NULL	NULL	DF	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DF of the bone is a rare , locally aggressive tumor .
	manualset3
257854	2	425988	7	NULL	NULL	NULL	NULL	 bone	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DF of the bone is a rare , locally aggressive tumor .
	manualset3
257855	3	425988	7	NULL	NULL	NULL	NULL	 locally aggressive tumor	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DF of the bone is a rare , locally aggressive tumor .
	manualset3
257858	1	425989	7	NULL	NULL	NULL	NULL	DFP	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DFP caused a reduction of the levels of ACh at 0.25 and 0.5 mg/kg .
	manualset3
257859	2	425989	7	NULL	NULL	NULL	NULL	reduction	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DFP caused a reduction of the levels of ACh at 0.25 and 0.5 mg/kg .
	manualset3
257860	3	425989	7	NULL	NULL	NULL	NULL	 levels	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DFP caused a reduction of the levels of ACh at 0.25 and 0.5 mg/kg .
	manualset3
257862	4	425989	7	NULL	NULL	NULL	NULL	ACh 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DFP caused a reduction of the levels of ACh at 0.25 and 0.5 mg/kg .
	manualset3
257864	5	425989	7	NULL	NULL	NULL	NULL	 0.25 mg/kg	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DFP caused a reduction of the levels of ACh at 0.25 and 0.5 mg/kg .
	manualset3
257867	6	425989	7	NULL	NULL	NULL	NULL	 0.5 mg/kg	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DFP caused a reduction of the levels of ACh at 0.25 and 0.5 mg/kg .
	manualset3
257868	1	425990	7	NULL	NULL	NULL	NULL	DIETARY DEPRIVATION	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DIETARY DEPRIVATION AND LIPOGENESIS IN A MODEL SEBACEOUS STRUCTURE .
	manualset3
257870	2	425990	7	NULL	NULL	NULL	NULL	LIPOGENESIS	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DIETARY DEPRIVATION AND LIPOGENESIS IN A MODEL SEBACEOUS STRUCTURE .
	manualset3
257871	3	425990	7	NULL	NULL	NULL	NULL	MODEL SEBACEOUS STRUCTURE	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DIETARY DEPRIVATION AND LIPOGENESIS IN A MODEL SEBACEOUS STRUCTURE .
	manualset3
257877	1	425991	7	NULL	NULL	NULL	NULL	DIMs	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DIMs are a structurally intriguing class of polyketide synthase-derived wax esters discovered over seventy years ago , yet , little was known until recently about their biosynthesis .
	manualset3
257879	2	425991	7	NULL	NULL	NULL	NULL	class	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DIMs are a structurally intriguing class of polyketide synthase-derived wax esters discovered over seventy years ago , yet , little was known until recently about their biosynthesis .
	manualset3
257880	3	425991	7	NULL	NULL	NULL	NULL	polyketide synthase-derived wax esters	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DIMs are a structurally intriguing class of polyketide synthase-derived wax esters discovered over seventy years ago , yet , little was known until recently about their biosynthesis .
	manualset3
257884	4	425991	7	NULL	NULL	NULL	NULL	 seventy years	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DIMs are a structurally intriguing class of polyketide synthase-derived wax esters discovered over seventy years ago , yet , little was known until recently about their biosynthesis .
	manualset3
257885	5	425991	7	NULL	NULL	NULL	NULL	 biosynthesis	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DIMs are a structurally intriguing class of polyketide synthase-derived wax esters discovered over seventy years ago , yet , little was known until recently about their biosynthesis .
	manualset3
257893	1	425992	7	NULL	NULL	NULL	NULL	DLLME 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DLLME is carried out with a throughput of 42 h ( -1 ) and DLLME for the extraction of benzo ( a ) pyrene and its subsequent chromatographic determination can be carried out with an analysis throughput of 7 h ( -1 ) .
	manualset3
257894	2	425992	7	NULL	NULL	NULL	NULL	42 h ( -1 )	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DLLME is carried out with a throughput of 42 h ( -1 ) and DLLME for the extraction of benzo ( a ) pyrene and its subsequent chromatographic determination can be carried out with an analysis throughput of 7 h ( -1 ) .
	manualset3
257896	3	425992	7	NULL	NULL	NULL	NULL	 DLLME 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DLLME is carried out with a throughput of 42 h ( -1 ) and DLLME for the extraction of benzo ( a ) pyrene and its subsequent chromatographic determination can be carried out with an analysis throughput of 7 h ( -1 ) .
	manualset3
257898	4	425992	7	NULL	NULL	NULL	NULL	extraction	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DLLME is carried out with a throughput of 42 h ( -1 ) and DLLME for the extraction of benzo ( a ) pyrene and its subsequent chromatographic determination can be carried out with an analysis throughput of 7 h ( -1 ) .
	manualset3
257899	5	425992	7	NULL	NULL	NULL	NULL	benzo ( a ) pyrene	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DLLME is carried out with a throughput of 42 h ( -1 ) and DLLME for the extraction of benzo ( a ) pyrene and its subsequent chromatographic determination can be carried out with an analysis throughput of 7 h ( -1 ) .
	manualset3
257901	6	425992	7	NULL	NULL	NULL	NULL	chromatographic determination	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DLLME is carried out with a throughput of 42 h ( -1 ) and DLLME for the extraction of benzo ( a ) pyrene and its subsequent chromatographic determination can be carried out with an analysis throughput of 7 h ( -1 ) .
	manualset3
257902	7	425992	7	NULL	NULL	NULL	NULL	analysis	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DLLME is carried out with a throughput of 42 h ( -1 ) and DLLME for the extraction of benzo ( a ) pyrene and its subsequent chromatographic determination can be carried out with an analysis throughput of 7 h ( -1 ) .
	manualset3
257906	8	425992	7	NULL	NULL	NULL	NULL	7 h ( -1 ) 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DLLME is carried out with a throughput of 42 h ( -1 ) and DLLME for the extraction of benzo ( a ) pyrene and its subsequent chromatographic determination can be carried out with an analysis throughput of 7 h ( -1 ) .
	manualset3
257999	1	425993	7	NULL	NULL	NULL	NULL	DM treatment 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DM treatment of the nuclei before UV irradiation results in extraction of the whole DM-sensitive H1 fraction ( ~ 25 % ) , which in this case is not stabilized in the nucleus .
	manualset3
258000	2	425993	7	NULL	NULL	NULL	NULL	nuclei	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DM treatment of the nuclei before UV irradiation results in extraction of the whole DM-sensitive H1 fraction ( ~ 25 % ) , which in this case is not stabilized in the nucleus .
	manualset3
258001	3	425993	7	NULL	NULL	NULL	NULL	UV irradiation	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DM treatment of the nuclei before UV irradiation results in extraction of the whole DM-sensitive H1 fraction ( ~ 25 % ) , which in this case is not stabilized in the nucleus .
	manualset3
258002	4	425993	7	NULL	NULL	NULL	NULL	extraction	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DM treatment of the nuclei before UV irradiation results in extraction of the whole DM-sensitive H1 fraction ( ~ 25 % ) , which in this case is not stabilized in the nucleus .
	manualset3
258003	5	425993	7	NULL	NULL	NULL	NULL	whole DM-sensitive H1 fraction	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DM treatment of the nuclei before UV irradiation results in extraction of the whole DM-sensitive H1 fraction ( ~ 25 % ) , which in this case is not stabilized in the nucleus .
	manualset3
258004	6	425993	7	NULL	NULL	NULL	NULL	25 %	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DM treatment of the nuclei before UV irradiation results in extraction of the whole DM-sensitive H1 fraction ( ~ 25 % ) , which in this case is not stabilized in the nucleus .
	manualset3
258005	7	425993	7	NULL	NULL	NULL	NULL	case	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DM treatment of the nuclei before UV irradiation results in extraction of the whole DM-sensitive H1 fraction ( ~ 25 % ) , which in this case is not stabilized in the nucleus .
	manualset3
258006	8	425993	7	NULL	NULL	NULL	NULL	 nucleus	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DM treatment of the nuclei before UV irradiation results in extraction of the whole DM-sensitive H1 fraction ( ~ 25 % ) , which in this case is not stabilized in the nucleus .
	manualset3
258016	1	425994	7	NULL	NULL	NULL	NULL	DMRT1	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DMRT1 is a conserved sex-determination gene that is upregulated in the male developing gonad in vertebrates , while DMRT7 is a mammal-specific spermatogenesis gene .
	manualset3
258017	2	425994	7	NULL	NULL	NULL	NULL	conserved sex-determination gene 	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DMRT1 is a conserved sex-determination gene that is upregulated in the male developing gonad in vertebrates , while DMRT7 is a mammal-specific spermatogenesis gene .
	manualset3
258031	3	425994	7	NULL	NULL	NULL	NULL	 male developing gonad	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DMRT1 is a conserved sex-determination gene that is upregulated in the male developing gonad in vertebrates , while DMRT7 is a mammal-specific spermatogenesis gene .
	manualset3
258032	4	425994	7	NULL	NULL	NULL	NULL	vertebrates	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DMRT1 is a conserved sex-determination gene that is upregulated in the male developing gonad in vertebrates , while DMRT7 is a mammal-specific spermatogenesis gene .
	manualset3
258033	5	425994	7	NULL	NULL	NULL	NULL	DMRT7	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DMRT1 is a conserved sex-determination gene that is upregulated in the male developing gonad in vertebrates , while DMRT7 is a mammal-specific spermatogenesis gene .
	manualset3
258034	6	425994	7	NULL	NULL	NULL	NULL	mammal-specific spermatogenesis gene	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DMRT1 is a conserved sex-determination gene that is upregulated in the male developing gonad in vertebrates , while DMRT7 is a mammal-specific spermatogenesis gene .
	manualset3
258035	1	425995	7	NULL	NULL	NULL	NULL	therapeutic improvement	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( A therapeutic improvement : second generation tyrosine kinase inhibitors ( TKI 2 ) in the treatment of chronic myelogenous leukemia ) .
	manualset3
258036	2	425995	7	NULL	NULL	NULL	NULL	second generation tyrosine kinase inhibitors ( TKI 2 )	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( A therapeutic improvement : second generation tyrosine kinase inhibitors ( TKI 2 ) in the treatment of chronic myelogenous leukemia ) .
	manualset3
258037	3	425995	7	NULL	NULL	NULL	NULL	treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( A therapeutic improvement : second generation tyrosine kinase inhibitors ( TKI 2 ) in the treatment of chronic myelogenous leukemia ) .
	manualset3
258038	4	425995	7	NULL	NULL	NULL	NULL	chronic myelogenous leukemia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( A therapeutic improvement : second generation tyrosine kinase inhibitors ( TKI 2 ) in the treatment of chronic myelogenous leukemia ) .
	manualset3
258039	1	425996	7	NULL	NULL	NULL	NULL	Microwave volumetry	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Microwave volumetry of the extremities : a technical measuring alternative to the noninvasive venous occlusion test ) .
	manualset3
258040	2	425996	7	NULL	NULL	NULL	NULL	extremities	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Microwave volumetry of the extremities : a technical measuring alternative to the noninvasive venous occlusion test ) .
	manualset3
258041	3	425996	7	NULL	NULL	NULL	NULL	 noninvasive venous occlusion test	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Microwave volumetry of the extremities : a technical measuring alternative to the noninvasive venous occlusion test ) .
	manualset3
258042	1	425997	7	NULL	NULL	NULL	NULL	DNA-DNA hybridization measurements	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA-DNA hybridization measurements showed low DNA relatedness ( 15-20 % ) between the isolate and its closest relatives .
	manualset3
258043	2	425997	7	NULL	NULL	NULL	NULL	low DNA relatedness	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA-DNA hybridization measurements showed low DNA relatedness ( 15-20 % ) between the isolate and its closest relatives .
	manualset3
258044	3	425997	7	NULL	NULL	NULL	NULL	15-20 %	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA-DNA hybridization measurements showed low DNA relatedness ( 15-20 % ) between the isolate and its closest relatives .
	manualset3
258045	4	425997	7	NULL	NULL	NULL	NULL	isolate	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA-DNA hybridization measurements showed low DNA relatedness ( 15-20 % ) between the isolate and its closest relatives .
	manualset3
258046	5	425997	7	NULL	NULL	NULL	NULL	closest relatives	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA-DNA hybridization measurements showed low DNA relatedness ( 15-20 % ) between the isolate and its closest relatives .
	manualset3
258047	1	425998	7	NULL	NULL	NULL	NULL	DNA-adduct levels 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA-adduct levels as a predictor of outcome for NSCLC patients receiving daily cisplatin and radiotherapy .
	manualset3
258048	2	425998	7	NULL	NULL	NULL	NULL	 predictor	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA-adduct levels as a predictor of outcome for NSCLC patients receiving daily cisplatin and radiotherapy .
	manualset3
258049	3	425998	7	NULL	NULL	NULL	NULL	 outcome	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA-adduct levels as a predictor of outcome for NSCLC patients receiving daily cisplatin and radiotherapy .
	manualset3
258050	4	425998	7	NULL	NULL	NULL	NULL	NSCLC patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA-adduct levels as a predictor of outcome for NSCLC patients receiving daily cisplatin and radiotherapy .
	manualset3
258051	5	425998	7	NULL	NULL	NULL	NULL	cisplatin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA-adduct levels as a predictor of outcome for NSCLC patients receiving daily cisplatin and radiotherapy .
	manualset3
258052	6	425998	7	NULL	NULL	NULL	NULL	radiotherapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA-adduct levels as a predictor of outcome for NSCLC patients receiving daily cisplatin and radiotherapy .
	manualset3
258053	1	425999	7	NULL	NULL	NULL	NULL	DNA-dependent RNA polymerases	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA-dependent RNA polymerases from Artemia salina .
	manualset3
258054	2	425999	7	NULL	NULL	NULL	NULL	Artemia salina	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA-dependent RNA polymerases from Artemia salina .
	manualset3
258055	1	426000	7	NULL	NULL	NULL	NULL	DNA adduct levels	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA adduct levels associated with p53 induction and delay of MCF-7 cells in S phase after exposure to benzo ( g ) chrysene dihydrodiol epoxide enantiomers .
	manualset3
258056	2	426000	7	NULL	NULL	NULL	NULL	p53 induction	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA adduct levels associated with p53 induction and delay of MCF-7 cells in S phase after exposure to benzo ( g ) chrysene dihydrodiol epoxide enantiomers .
	manualset3
258057	3	426000	7	NULL	NULL	NULL	NULL	delay	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA adduct levels associated with p53 induction and delay of MCF-7 cells in S phase after exposure to benzo ( g ) chrysene dihydrodiol epoxide enantiomers .
	manualset3
258058	4	426000	7	NULL	NULL	NULL	NULL	MCF-7 cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA adduct levels associated with p53 induction and delay of MCF-7 cells in S phase after exposure to benzo ( g ) chrysene dihydrodiol epoxide enantiomers .
	manualset3
258059	5	426000	7	NULL	NULL	NULL	NULL	S phase	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA adduct levels associated with p53 induction and delay of MCF-7 cells in S phase after exposure to benzo ( g ) chrysene dihydrodiol epoxide enantiomers .
	manualset3
258060	6	426000	7	NULL	NULL	NULL	NULL	exposure	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA adduct levels associated with p53 induction and delay of MCF-7 cells in S phase after exposure to benzo ( g ) chrysene dihydrodiol epoxide enantiomers .
	manualset3
258061	7	426000	7	NULL	NULL	NULL	NULL	 benzo ( g ) chrysene dihydrodiol epoxide enantiomers	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA adduct levels associated with p53 induction and delay of MCF-7 cells in S phase after exposure to benzo ( g ) chrysene dihydrodiol epoxide enantiomers .
	manualset3
258062	1	426001	7	NULL	NULL	NULL	NULL	DNA damage	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA damage by hydroquinone in human white blood cells : analysis by alkaline single-cell gel electrophoresis .
	manualset3
258063	2	426001	7	NULL	NULL	NULL	NULL	hydroquinone	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA damage by hydroquinone in human white blood cells : analysis by alkaline single-cell gel electrophoresis .
	manualset3
258064	3	426001	7	NULL	NULL	NULL	NULL	human white blood cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA damage by hydroquinone in human white blood cells : analysis by alkaline single-cell gel electrophoresis .
	manualset3
258065	4	426001	7	NULL	NULL	NULL	NULL	analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA damage by hydroquinone in human white blood cells : analysis by alkaline single-cell gel electrophoresis .
	manualset3
258066	5	426001	7	NULL	NULL	NULL	NULL	alkaline single-cell gel electrophoresis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA damage by hydroquinone in human white blood cells : analysis by alkaline single-cell gel electrophoresis .
	manualset3
258067	1	426002	7	NULL	NULL	NULL	NULL	DNA damage	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA damage was caused by ionizing radiation ( IR ) and cytotoxic drugs , cultured tissues were treated with ATM and DNA-PK inhibitors , and DDR was assessed by phosphorylation of ATM and its targets H2AX and KAP1 , a heterochromatin binding protein .
	manualset3
258068	2	426002	7	NULL	NULL	NULL	NULL	ionizing radiation ( IR )	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA damage was caused by ionizing radiation ( IR ) and cytotoxic drugs , cultured tissues were treated with ATM and DNA-PK inhibitors , and DDR was assessed by phosphorylation of ATM and its targets H2AX and KAP1 , a heterochromatin binding protein .
	manualset3
258069	3	426002	7	NULL	NULL	NULL	NULL	cytotoxic drugs	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA damage was caused by ionizing radiation ( IR ) and cytotoxic drugs , cultured tissues were treated with ATM and DNA-PK inhibitors , and DDR was assessed by phosphorylation of ATM and its targets H2AX and KAP1 , a heterochromatin binding protein .
	manualset3
258070	4	426002	7	NULL	NULL	NULL	NULL	cultured tissues	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA damage was caused by ionizing radiation ( IR ) and cytotoxic drugs , cultured tissues were treated with ATM and DNA-PK inhibitors , and DDR was assessed by phosphorylation of ATM and its targets H2AX and KAP1 , a heterochromatin binding protein .
	manualset3
258071	5	426002	7	NULL	NULL	NULL	NULL	ATM inhibitors	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA damage was caused by ionizing radiation ( IR ) and cytotoxic drugs , cultured tissues were treated with ATM and DNA-PK inhibitors , and DDR was assessed by phosphorylation of ATM and its targets H2AX and KAP1 , a heterochromatin binding protein .
	manualset3
258072	6	426002	7	NULL	NULL	NULL	NULL	DNA-PK inhibitors	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA damage was caused by ionizing radiation ( IR ) and cytotoxic drugs , cultured tissues were treated with ATM and DNA-PK inhibitors , and DDR was assessed by phosphorylation of ATM and its targets H2AX and KAP1 , a heterochromatin binding protein .
	manualset3
258073	7	426002	7	NULL	NULL	NULL	NULL	DDR	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA damage was caused by ionizing radiation ( IR ) and cytotoxic drugs , cultured tissues were treated with ATM and DNA-PK inhibitors , and DDR was assessed by phosphorylation of ATM and its targets H2AX and KAP1 , a heterochromatin binding protein .
	manualset3
258074	8	426002	7	NULL	NULL	NULL	NULL	phosphorylation 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA damage was caused by ionizing radiation ( IR ) and cytotoxic drugs , cultured tissues were treated with ATM and DNA-PK inhibitors , and DDR was assessed by phosphorylation of ATM and its targets H2AX and KAP1 , a heterochromatin binding protein .
	manualset3
258075	9	426002	7	NULL	NULL	NULL	NULL	ATM 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA damage was caused by ionizing radiation ( IR ) and cytotoxic drugs , cultured tissues were treated with ATM and DNA-PK inhibitors , and DDR was assessed by phosphorylation of ATM and its targets H2AX and KAP1 , a heterochromatin binding protein .
	manualset3
258076	10	426002	7	NULL	NULL	NULL	NULL	 targets	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA damage was caused by ionizing radiation ( IR ) and cytotoxic drugs , cultured tissues were treated with ATM and DNA-PK inhibitors , and DDR was assessed by phosphorylation of ATM and its targets H2AX and KAP1 , a heterochromatin binding protein .
	manualset3
258077	11	426002	7	NULL	NULL	NULL	NULL	H2AX 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA damage was caused by ionizing radiation ( IR ) and cytotoxic drugs , cultured tissues were treated with ATM and DNA-PK inhibitors , and DDR was assessed by phosphorylation of ATM and its targets H2AX and KAP1 , a heterochromatin binding protein .
	manualset3
258078	12	426002	7	NULL	NULL	NULL	NULL	KAP1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA damage was caused by ionizing radiation ( IR ) and cytotoxic drugs , cultured tissues were treated with ATM and DNA-PK inhibitors , and DDR was assessed by phosphorylation of ATM and its targets H2AX and KAP1 , a heterochromatin binding protein .
	manualset3
258079	13	426002	7	NULL	NULL	NULL	NULL	heterochromatin binding protein	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA damage was caused by ionizing radiation ( IR ) and cytotoxic drugs , cultured tissues were treated with ATM and DNA-PK inhibitors , and DDR was assessed by phosphorylation of ATM and its targets H2AX and KAP1 , a heterochromatin binding protein .
	manualset3
258080	1	426003	7	NULL	NULL	NULL	NULL	DNA fingerprinting 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA fingerprinting using a nonisotopically labeled minisatellite probe provided a valuable technique for genetic monitoring/quality control of laboratory rodents .
	manualset3
258081	2	426003	7	NULL	NULL	NULL	NULL	nonisotopically labeled minisatellite probe	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA fingerprinting using a nonisotopically labeled minisatellite probe provided a valuable technique for genetic monitoring/quality control of laboratory rodents .
	manualset3
258082	3	426003	7	NULL	NULL	NULL	NULL	 valuable technique	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA fingerprinting using a nonisotopically labeled minisatellite probe provided a valuable technique for genetic monitoring/quality control of laboratory rodents .
	manualset3
258083	4	426003	7	NULL	NULL	NULL	NULL	 genetic monitoring	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA fingerprinting using a nonisotopically labeled minisatellite probe provided a valuable technique for genetic monitoring/quality control of laboratory rodents .
	manualset3
258084	5	426003	7	NULL	NULL	NULL	NULL	quality control 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA fingerprinting using a nonisotopically labeled minisatellite probe provided a valuable technique for genetic monitoring/quality control of laboratory rodents .
	manualset3
258085	6	426003	7	NULL	NULL	NULL	NULL	laboratory rodents	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA fingerprinting using a nonisotopically labeled minisatellite probe provided a valuable technique for genetic monitoring/quality control of laboratory rodents .
	manualset3
258086	1	426004	7	NULL	NULL	NULL	NULL	DNA gel blot analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA gel blot analysis with the cloned specifically unmethylated regions ( SUMs ) showed that some SUMs were methylated differentially in bacteroids compared to free-living bacteria .
	manualset3
258087	2	426004	7	NULL	NULL	NULL	NULL	specifically unmethylated regions ( SUMs )	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA gel blot analysis with the cloned specifically unmethylated regions ( SUMs ) showed that some SUMs were methylated differentially in bacteroids compared to free-living bacteria .
	manualset3
258088	3	426004	7	NULL	NULL	NULL	NULL	SUMs	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA gel blot analysis with the cloned specifically unmethylated regions ( SUMs ) showed that some SUMs were methylated differentially in bacteroids compared to free-living bacteria .
	manualset3
258089	4	426004	7	NULL	NULL	NULL	NULL	 bacteroids	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA gel blot analysis with the cloned specifically unmethylated regions ( SUMs ) showed that some SUMs were methylated differentially in bacteroids compared to free-living bacteria .
	manualset3
258090	5	426004	7	NULL	NULL	NULL	NULL	free-living bacteria	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA gel blot analysis with the cloned specifically unmethylated regions ( SUMs ) showed that some SUMs were methylated differentially in bacteroids compared to free-living bacteria .
	manualset3
258091	1	426005	7	NULL	NULL	NULL	NULL	DNA hypomethylation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA hypomethylation and germ cell-specific expression of testis-specific H2B histone gene .
	manualset3
258092	2	426005	7	NULL	NULL	NULL	NULL	germ cell-specific expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA hypomethylation and germ cell-specific expression of testis-specific H2B histone gene .
	manualset3
258093	3	426005	7	NULL	NULL	NULL	NULL	testis-specific H2B histone gene	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA hypomethylation and germ cell-specific expression of testis-specific H2B histone gene .
	manualset3
258094	1	426006	7	NULL	NULL	NULL	NULL	DNA ligase III 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA ligase III is recruited to DNA strand breaks by a zinc finger motif homologous to that of poly ( ADP-ribose ) polymerase .
	manualset3
258095	2	426006	7	NULL	NULL	NULL	NULL	DNA strand breaks	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA ligase III is recruited to DNA strand breaks by a zinc finger motif homologous to that of poly ( ADP-ribose ) polymerase .
	manualset3
258096	3	426006	7	NULL	NULL	NULL	NULL	zinc finger motif	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA ligase III is recruited to DNA strand breaks by a zinc finger motif homologous to that of poly ( ADP-ribose ) polymerase .
	manualset3
258097	4	426006	7	NULL	NULL	NULL	NULL	poly ( ADP-ribose ) polymerase	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA ligase III is recruited to DNA strand breaks by a zinc finger motif homologous to that of poly ( ADP-ribose ) polymerase .
	manualset3
258098	1	426007	7	NULL	NULL	NULL	NULL	DNA methylation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA methylation has been shown to be altered in response to toxicants and heavy metals , although investigation of other epigenetic mechanisms is only beginning .
	manualset3
258099	2	426007	7	NULL	NULL	NULL	NULL	toxicants	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA methylation has been shown to be altered in response to toxicants and heavy metals , although investigation of other epigenetic mechanisms is only beginning .
	manualset3
258100	3	426007	7	NULL	NULL	NULL	NULL	heavy metals	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA methylation has been shown to be altered in response to toxicants and heavy metals , although investigation of other epigenetic mechanisms is only beginning .
	manualset3
258101	4	426007	7	NULL	NULL	NULL	NULL	investigation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA methylation has been shown to be altered in response to toxicants and heavy metals , although investigation of other epigenetic mechanisms is only beginning .
	manualset3
258102	5	426007	7	NULL	NULL	NULL	NULL	epigenetic mechanisms	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA methylation has been shown to be altered in response to toxicants and heavy metals , although investigation of other epigenetic mechanisms is only beginning .
	manualset3
258103	6	426007	7	NULL	NULL	NULL	NULL	beginning	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA methylation has been shown to be altered in response to toxicants and heavy metals , although investigation of other epigenetic mechanisms is only beginning .
	manualset3
258104	1	426008	7	NULL	NULL	NULL	NULL	DNA probes	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA probes derived from the Y chromosome have been used to determine fetal sex .
	manualset3
258105	2	426008	7	NULL	NULL	NULL	NULL	 Y chromosome	Chromosome												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA probes derived from the Y chromosome have been used to determine fetal sex .
	manualset3
258106	3	426008	7	NULL	NULL	NULL	NULL	fetal sex	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA probes derived from the Y chromosome have been used to determine fetal sex .
	manualset3
258107	1	426009	7	NULL	NULL	NULL	NULL	DNA sequence analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA sequence analysis of a 3213 bp BamHI-ClaI fragment revealed that three open reading frames ( ORFs ) were encoded in the same orientation .
	manualset3
258108	2	426009	7	NULL	NULL	NULL	NULL	3213 bp BamHI-ClaI fragment	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA sequence analysis of a 3213 bp BamHI-ClaI fragment revealed that three open reading frames ( ORFs ) were encoded in the same orientation .
	manualset3
258109	3	426009	7	NULL	NULL	NULL	NULL	three open reading frames ( ORFs )	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA sequence analysis of a 3213 bp BamHI-ClaI fragment revealed that three open reading frames ( ORFs ) were encoded in the same orientation .
	manualset3
258110	4	426009	7	NULL	NULL	NULL	NULL	same orientation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA sequence analysis of a 3213 bp BamHI-ClaI fragment revealed that three open reading frames ( ORFs ) were encoded in the same orientation .
	manualset3
258111	1	426010	7	NULL	NULL	NULL	NULL	DNA sequencing 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA sequencing revealed seven different glucose-6-phosphate dehydrogenase ( G6PD ) mutations in G6PD deficient subjects from 10 Polish families .
	manualset3
258112	2	426010	7	NULL	NULL	NULL	NULL	seven different glucose-6-phosphate dehydrogenase ( G6PD ) mutations	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA sequencing revealed seven different glucose-6-phosphate dehydrogenase ( G6PD ) mutations in G6PD deficient subjects from 10 Polish families .
	manualset3
258113	3	426010	7	NULL	NULL	NULL	NULL	G6PD deficient subjects	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA sequencing revealed seven different glucose-6-phosphate dehydrogenase ( G6PD ) mutations in G6PD deficient subjects from 10 Polish families .
	manualset3
258114	4	426010	7	NULL	NULL	NULL	NULL	10 Polish families 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA sequencing revealed seven different glucose-6-phosphate dehydrogenase ( G6PD ) mutations in G6PD deficient subjects from 10 Polish families .
	manualset3
258115	1	426011	7	NULL	NULL	NULL	NULL	Military school 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Military school of aviation medicine ) .
	manualset3
258116	2	426011	7	NULL	NULL	NULL	NULL	 aviation medicine	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Military school of aviation medicine ) .
	manualset3
258117	1	426012	7	NULL	NULL	NULL	NULL	DNA synthesis	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA synthesis in prothoracic gland cells of the silkworm , Bombyx mori , was studied immunocytochemically after in vivo labeling with 5-bromo-2 ' - deoxyuridine ( BrdU ) , and its developmental changes during the 3rd , 4th , and last larval instars were examined .
	manualset3
258118	2	426012	7	NULL	NULL	NULL	NULL	prothoracic gland cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA synthesis in prothoracic gland cells of the silkworm , Bombyx mori , was studied immunocytochemically after in vivo labeling with 5-bromo-2 ' - deoxyuridine ( BrdU ) , and its developmental changes during the 3rd , 4th , and last larval instars were examined .
	manualset3
258119	3	426012	7	NULL	NULL	NULL	NULL	 silkworm	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA synthesis in prothoracic gland cells of the silkworm , Bombyx mori , was studied immunocytochemically after in vivo labeling with 5-bromo-2 ' - deoxyuridine ( BrdU ) , and its developmental changes during the 3rd , 4th , and last larval instars were examined .
	manualset3
258120	4	426012	7	NULL	NULL	NULL	NULL	Bombyx mori	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA synthesis in prothoracic gland cells of the silkworm , Bombyx mori , was studied immunocytochemically after in vivo labeling with 5-bromo-2 ' - deoxyuridine ( BrdU ) , and its developmental changes during the 3rd , 4th , and last larval instars were examined .
	manualset3
258121	5	426012	7	NULL	NULL	NULL	NULL	in vivo labeling	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA synthesis in prothoracic gland cells of the silkworm , Bombyx mori , was studied immunocytochemically after in vivo labeling with 5-bromo-2 ' - deoxyuridine ( BrdU ) , and its developmental changes during the 3rd , 4th , and last larval instars were examined .
	manualset3
258122	6	426012	7	NULL	NULL	NULL	NULL	5-bromo-2 ' - deoxyuridine ( BrdU )	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA synthesis in prothoracic gland cells of the silkworm , Bombyx mori , was studied immunocytochemically after in vivo labeling with 5-bromo-2 ' - deoxyuridine ( BrdU ) , and its developmental changes during the 3rd , 4th , and last larval instars were examined .
	manualset3
258123	7	426012	7	NULL	NULL	NULL	NULL	developmental changes	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA synthesis in prothoracic gland cells of the silkworm , Bombyx mori , was studied immunocytochemically after in vivo labeling with 5-bromo-2 ' - deoxyuridine ( BrdU ) , and its developmental changes during the 3rd , 4th , and last larval instars were examined .
	manualset3
258124	8	426012	7	NULL	NULL	NULL	NULL	3rd larval instars	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA synthesis in prothoracic gland cells of the silkworm , Bombyx mori , was studied immunocytochemically after in vivo labeling with 5-bromo-2 ' - deoxyuridine ( BrdU ) , and its developmental changes during the 3rd , 4th , and last larval instars were examined .
	manualset3
258125	9	426012	7	NULL	NULL	NULL	NULL	4th  larval instars	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA synthesis in prothoracic gland cells of the silkworm , Bombyx mori , was studied immunocytochemically after in vivo labeling with 5-bromo-2 ' - deoxyuridine ( BrdU ) , and its developmental changes during the 3rd , 4th , and last larval instars were examined .
	manualset3
258126	10	426012	7	NULL	NULL	NULL	NULL	last larval instars	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA synthesis in prothoracic gland cells of the silkworm , Bombyx mori , was studied immunocytochemically after in vivo labeling with 5-bromo-2 ' - deoxyuridine ( BrdU ) , and its developmental changes during the 3rd , 4th , and last larval instars were examined .
	manualset3
258127	1	426013	7	NULL	NULL	NULL	NULL	DNA topoisomerases	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA topoisomerases are believed to promote transcription by removing excessive DNA supercoils produced during elongation .
	manualset3
258128	2	426013	7	NULL	NULL	NULL	NULL	transcription	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA topoisomerases are believed to promote transcription by removing excessive DNA supercoils produced during elongation .
	manualset3
258129	3	426013	7	NULL	NULL	NULL	NULL	DNA supercoils	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA topoisomerases are believed to promote transcription by removing excessive DNA supercoils produced during elongation .
	manualset3
258130	4	426013	7	NULL	NULL	NULL	NULL	elongation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA topoisomerases are believed to promote transcription by removing excessive DNA supercoils produced during elongation .
	manualset3
258131	1	426014	7	NULL	NULL	NULL	NULL	DNA	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA was extracted from these specimens and typing of C. trachomatis serovars was performed by the polymerase chain reaction-restriction fragment length polymorphism method .
	manualset3
258132	2	426014	7	NULL	NULL	NULL	NULL	specimens	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA was extracted from these specimens and typing of C. trachomatis serovars was performed by the polymerase chain reaction-restriction fragment length polymorphism method .
	manualset3
258133	3	426014	7	NULL	NULL	NULL	NULL	 typing 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA was extracted from these specimens and typing of C. trachomatis serovars was performed by the polymerase chain reaction-restriction fragment length polymorphism method .
	manualset3
258134	4	426014	7	NULL	NULL	NULL	NULL	C. trachomatis serovars	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA was extracted from these specimens and typing of C. trachomatis serovars was performed by the polymerase chain reaction-restriction fragment length polymorphism method .
	manualset3
258135	5	426014	7	NULL	NULL	NULL	NULL	polymerase chain reaction-restriction fragment length polymorphism method	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA was extracted from these specimens and typing of C. trachomatis serovars was performed by the polymerase chain reaction-restriction fragment length polymorphism method .
	manualset3
258136	1	426015	7	NULL	NULL	NULL	NULL	DNA	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA was isolated and detected by Southern blot from since 50 microliters dried bloodstains ( HinfI , G3 , MS1 , MS31 ) , from various specimen bloodstains and from dried semen stains .
	manualset3
258137	2	426015	7	NULL	NULL	NULL	NULL	Southern blot	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA was isolated and detected by Southern blot from since 50 microliters dried bloodstains ( HinfI , G3 , MS1 , MS31 ) , from various specimen bloodstains and from dried semen stains .
	manualset3
258138	3	426015	7	NULL	NULL	NULL	NULL	50 microliters dried bloodstains	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA was isolated and detected by Southern blot from since 50 microliters dried bloodstains ( HinfI , G3 , MS1 , MS31 ) , from various specimen bloodstains and from dried semen stains .
	manualset3
258139	4	426015	7	NULL	NULL	NULL	NULL	HinfI	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA was isolated and detected by Southern blot from since 50 microliters dried bloodstains ( HinfI , G3 , MS1 , MS31 ) , from various specimen bloodstains and from dried semen stains .
	manualset3
258140	5	426015	7	NULL	NULL	NULL	NULL	G3	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA was isolated and detected by Southern blot from since 50 microliters dried bloodstains ( HinfI , G3 , MS1 , MS31 ) , from various specimen bloodstains and from dried semen stains .
	manualset3
258141	6	426015	7	NULL	NULL	NULL	NULL	MS1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA was isolated and detected by Southern blot from since 50 microliters dried bloodstains ( HinfI , G3 , MS1 , MS31 ) , from various specimen bloodstains and from dried semen stains .
	manualset3
258142	7	426015	7	NULL	NULL	NULL	NULL	MS31	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA was isolated and detected by Southern blot from since 50 microliters dried bloodstains ( HinfI , G3 , MS1 , MS31 ) , from various specimen bloodstains and from dried semen stains .
	manualset3
258143	8	426015	7	NULL	NULL	NULL	NULL	specimen bloodstains	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA was isolated and detected by Southern blot from since 50 microliters dried bloodstains ( HinfI , G3 , MS1 , MS31 ) , from various specimen bloodstains and from dried semen stains .
	manualset3
258144	9	426015	7	NULL	NULL	NULL	NULL	 dried semen stains	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNA was isolated and detected by Southern blot from since 50 microliters dried bloodstains ( HinfI , G3 , MS1 , MS31 ) , from various specimen bloodstains and from dried semen stains .
	manualset3
258438	1	426016	7	NULL	NULL	NULL	NULL	DNAs	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNAs isolated from tumors were examined by means of a RNase protection analysis , coupled with the polymerase chain reaction followed by DNA sequencing of the polymerase chain reaction products .
	manualset3
258440	2	426016	7	NULL	NULL	NULL	NULL	 tumors	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNAs isolated from tumors were examined by means of a RNase protection analysis , coupled with the polymerase chain reaction followed by DNA sequencing of the polymerase chain reaction products .
	manualset3
258442	3	426016	7	NULL	NULL	NULL	NULL	RNase protection analysis	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNAs isolated from tumors were examined by means of a RNase protection analysis , coupled with the polymerase chain reaction followed by DNA sequencing of the polymerase chain reaction products .
	manualset3
258443	4	426016	7	NULL	NULL	NULL	NULL	polymerase chain reaction	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNAs isolated from tumors were examined by means of a RNase protection analysis , coupled with the polymerase chain reaction followed by DNA sequencing of the polymerase chain reaction products .
	manualset3
258445	5	426016	7	NULL	NULL	NULL	NULL	DNA sequencing	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNAs isolated from tumors were examined by means of a RNase protection analysis , coupled with the polymerase chain reaction followed by DNA sequencing of the polymerase chain reaction products .
	manualset3
258446	6	426016	7	NULL	NULL	NULL	NULL	polymerase chain reaction products	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNAs isolated from tumors were examined by means of a RNase protection analysis , coupled with the polymerase chain reaction followed by DNA sequencing of the polymerase chain reaction products .
	manualset3
258448	1	426017	7	NULL	NULL	NULL	NULL	DNAzyme 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNAzyme for TGF-beta suppressed extracellular matrix accumulation in experimental glomerulonephritis .
	manualset3
258450	2	426017	7	NULL	NULL	NULL	NULL	 TGF-beta suppressed extracellular matrix accumulation 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNAzyme for TGF-beta suppressed extracellular matrix accumulation in experimental glomerulonephritis .
	manualset3
258452	3	426017	7	NULL	NULL	NULL	NULL	experimental glomerulonephritis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNAzyme for TGF-beta suppressed extracellular matrix accumulation in experimental glomerulonephritis .
	manualset3
258454	1	426018	7	NULL	NULL	NULL	NULL	DNAzymes	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNAzymes are catalytically active DNA molecules that use metal cofactors for their enzymatic functions .
	manualset3
258457	2	426018	7	NULL	NULL	NULL	NULL	catalytically active DNA molecules	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNAzymes are catalytically active DNA molecules that use metal cofactors for their enzymatic functions .
	manualset3
258459	3	426018	7	NULL	NULL	NULL	NULL	 metal cofactors	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNAzymes are catalytically active DNA molecules that use metal cofactors for their enzymatic functions .
	manualset3
258461	4	426018	7	NULL	NULL	NULL	NULL	enzymatic functions	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNAzymes are catalytically active DNA molecules that use metal cofactors for their enzymatic functions .
	manualset3
258464	1	426019	7	NULL	NULL	NULL	NULL	DNase I footprinting analysis	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNase I footprinting analysis has defined the FruR binding site .
	manualset3
258465	2	426019	7	NULL	NULL	NULL	NULL	FruR binding site	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DNase I footprinting analysis has defined the FruR binding site .
	manualset3
258472	1	426020	7	NULL	NULL	NULL	NULL	DOC	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DOC also induced recruitment of the histone acetyltransferase p300 to the TAT-GRE as efficiently as DEX .
	manualset3
258473	2	426020	7	NULL	NULL	NULL	NULL	recruitment 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DOC also induced recruitment of the histone acetyltransferase p300 to the TAT-GRE as efficiently as DEX .
	manualset3
258475	3	426020	7	NULL	NULL	NULL	NULL	histone acetyltransferase p300	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DOC also induced recruitment of the histone acetyltransferase p300 to the TAT-GRE as efficiently as DEX .
	manualset3
258482	4	426020	7	NULL	NULL	NULL	NULL	TAT-GRE	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DOC also induced recruitment of the histone acetyltransferase p300 to the TAT-GRE as efficiently as DEX .
	manualset3
258484	5	426020	7	NULL	NULL	NULL	NULL	DEX	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DOC also induced recruitment of the histone acetyltransferase p300 to the TAT-GRE as efficiently as DEX .
	manualset3
258529	1	426021	7	NULL	NULL	NULL	NULL	DON	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DON was found to readily induce phosphorylation of JNK 1/2 , ERK 1/2 , and p38 in the murine macrophage RAW 264.7 cell line , within 5 min of culture addition , in a concentration-dependent fashion .
	manualset3
258530	2	426021	7	NULL	NULL	NULL	NULL	phosphorylation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DON was found to readily induce phosphorylation of JNK 1/2 , ERK 1/2 , and p38 in the murine macrophage RAW 264.7 cell line , within 5 min of culture addition , in a concentration-dependent fashion .
	manualset3
258531	3	426021	7	NULL	NULL	NULL	NULL	JNK 1/2	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DON was found to readily induce phosphorylation of JNK 1/2 , ERK 1/2 , and p38 in the murine macrophage RAW 264.7 cell line , within 5 min of culture addition , in a concentration-dependent fashion .
	manualset3
258532	4	426021	7	NULL	NULL	NULL	NULL	ERK 1/2	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DON was found to readily induce phosphorylation of JNK 1/2 , ERK 1/2 , and p38 in the murine macrophage RAW 264.7 cell line , within 5 min of culture addition , in a concentration-dependent fashion .
	manualset3
258533	5	426021	7	NULL	NULL	NULL	NULL	 p38	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DON was found to readily induce phosphorylation of JNK 1/2 , ERK 1/2 , and p38 in the murine macrophage RAW 264.7 cell line , within 5 min of culture addition , in a concentration-dependent fashion .
	manualset3
258534	6	426021	7	NULL	NULL	NULL	NULL	murine macrophage RAW 264.7 cell line	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DON was found to readily induce phosphorylation of JNK 1/2 , ERK 1/2 , and p38 in the murine macrophage RAW 264.7 cell line , within 5 min of culture addition , in a concentration-dependent fashion .
	manualset3
258535	7	426021	7	NULL	NULL	NULL	NULL	5 min	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DON was found to readily induce phosphorylation of JNK 1/2 , ERK 1/2 , and p38 in the murine macrophage RAW 264.7 cell line , within 5 min of culture addition , in a concentration-dependent fashion .
	manualset3
258536	8	426021	7	NULL	NULL	NULL	NULL	 culture	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DON was found to readily induce phosphorylation of JNK 1/2 , ERK 1/2 , and p38 in the murine macrophage RAW 264.7 cell line , within 5 min of culture addition , in a concentration-dependent fashion .
	manualset3
258537	9	426021	7	NULL	NULL	NULL	NULL	concentration-dependent fashion	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DON was found to readily induce phosphorylation of JNK 1/2 , ERK 1/2 , and p38 in the murine macrophage RAW 264.7 cell line , within 5 min of culture addition , in a concentration-dependent fashion .
	manualset3
258538	1	426022	7	NULL	NULL	NULL	NULL	Molecular aspects	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Molecular aspects of glucocorticoid regulation of cardiac metabolism ) .
	manualset3
258539	2	426022	7	NULL	NULL	NULL	NULL	glucocorticoid regulation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Molecular aspects of glucocorticoid regulation of cardiac metabolism ) .
	manualset3
258540	3	426022	7	NULL	NULL	NULL	NULL	cardiac metabolism	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Molecular aspects of glucocorticoid regulation of cardiac metabolism ) .
	manualset3
258541	1	426023	7	NULL	NULL	NULL	NULL	DSC	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DSC and rheometric studies are used to follow thermogelation , a process involving hydrophobic interaction between partly hydrated polymeric chains .
	manualset3
258542	2	426023	7	NULL	NULL	NULL	NULL	rheometric studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DSC and rheometric studies are used to follow thermogelation , a process involving hydrophobic interaction between partly hydrated polymeric chains .
	manualset3
258543	3	426023	7	NULL	NULL	NULL	NULL	thermogelation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DSC and rheometric studies are used to follow thermogelation , a process involving hydrophobic interaction between partly hydrated polymeric chains .
	manualset3
258544	4	426023	7	NULL	NULL	NULL	NULL	process	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DSC and rheometric studies are used to follow thermogelation , a process involving hydrophobic interaction between partly hydrated polymeric chains .
	manualset3
258545	5	426023	7	NULL	NULL	NULL	NULL	hydrophobic interaction	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DSC and rheometric studies are used to follow thermogelation , a process involving hydrophobic interaction between partly hydrated polymeric chains .
	manualset3
258546	6	426023	7	NULL	NULL	NULL	NULL	partly hydrated polymeric chains 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DSC and rheometric studies are used to follow thermogelation , a process involving hydrophobic interaction between partly hydrated polymeric chains .
	manualset3
258547	1	426024	7	NULL	NULL	NULL	NULL	DSIF	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DSIF and NELF interact with RNA polymerase II elongation complex and HIV-1 Tat stimulates P-TEFb-mediated phosphorylation of RNA polymerase II and DSIF during transcription elongation .
	manualset3
258548	2	426024	7	NULL	NULL	NULL	NULL	NELF	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DSIF and NELF interact with RNA polymerase II elongation complex and HIV-1 Tat stimulates P-TEFb-mediated phosphorylation of RNA polymerase II and DSIF during transcription elongation .
	manualset3
258549	3	426024	7	NULL	NULL	NULL	NULL	RNA polymerase II elongation complex	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DSIF and NELF interact with RNA polymerase II elongation complex and HIV-1 Tat stimulates P-TEFb-mediated phosphorylation of RNA polymerase II and DSIF during transcription elongation .
	manualset3
258550	4	426024	7	NULL	NULL	NULL	NULL	 HIV-1 Tat	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DSIF and NELF interact with RNA polymerase II elongation complex and HIV-1 Tat stimulates P-TEFb-mediated phosphorylation of RNA polymerase II and DSIF during transcription elongation .
	manualset3
258551	5	426024	7	NULL	NULL	NULL	NULL	P-TEFb-mediated phosphorylation 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DSIF and NELF interact with RNA polymerase II elongation complex and HIV-1 Tat stimulates P-TEFb-mediated phosphorylation of RNA polymerase II and DSIF during transcription elongation .
	manualset3
258552	6	426024	7	NULL	NULL	NULL	NULL	RNA polymerase II 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DSIF and NELF interact with RNA polymerase II elongation complex and HIV-1 Tat stimulates P-TEFb-mediated phosphorylation of RNA polymerase II and DSIF during transcription elongation .
	manualset3
258553	7	426024	7	NULL	NULL	NULL	NULL	DSIF	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DSIF and NELF interact with RNA polymerase II elongation complex and HIV-1 Tat stimulates P-TEFb-mediated phosphorylation of RNA polymerase II and DSIF during transcription elongation .
	manualset3
258554	8	426024	7	NULL	NULL	NULL	NULL	transcription elongation 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DSIF and NELF interact with RNA polymerase II elongation complex and HIV-1 Tat stimulates P-TEFb-mediated phosphorylation of RNA polymerase II and DSIF during transcription elongation .
	manualset3
258555	1	426025	7	NULL	NULL	NULL	NULL	DSZ cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DSZ cells grown in liquid medium with SZ ( in 10 mM ethanol ) as carbon source mineralized 71.6 + / -1.3 % of 0.025 mM SZ with a yield of 4.6 + / -0.3 microg cell dry weight mmol ( -1 ) carbon .
	manualset3
258556	2	426025	7	NULL	NULL	NULL	NULL	liquid medium	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DSZ cells grown in liquid medium with SZ ( in 10 mM ethanol ) as carbon source mineralized 71.6 + / -1.3 % of 0.025 mM SZ with a yield of 4.6 + / -0.3 microg cell dry weight mmol ( -1 ) carbon .
	manualset3
258557	3	426025	7	NULL	NULL	NULL	NULL	SZ	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DSZ cells grown in liquid medium with SZ ( in 10 mM ethanol ) as carbon source mineralized 71.6 + / -1.3 % of 0.025 mM SZ with a yield of 4.6 + / -0.3 microg cell dry weight mmol ( -1 ) carbon .
	manualset3
258558	4	426025	7	NULL	NULL	NULL	NULL	10 mM 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DSZ cells grown in liquid medium with SZ ( in 10 mM ethanol ) as carbon source mineralized 71.6 + / -1.3 % of 0.025 mM SZ with a yield of 4.6 + / -0.3 microg cell dry weight mmol ( -1 ) carbon .
	manualset3
258559	5	426025	7	NULL	NULL	NULL	NULL	ethanol	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DSZ cells grown in liquid medium with SZ ( in 10 mM ethanol ) as carbon source mineralized 71.6 + / -1.3 % of 0.025 mM SZ with a yield of 4.6 + / -0.3 microg cell dry weight mmol ( -1 ) carbon .
	manualset3
258560	6	426025	7	NULL	NULL	NULL	NULL	carbon source	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DSZ cells grown in liquid medium with SZ ( in 10 mM ethanol ) as carbon source mineralized 71.6 + / -1.3 % of 0.025 mM SZ with a yield of 4.6 + / -0.3 microg cell dry weight mmol ( -1 ) carbon .
	manualset3
258561	7	426025	7	NULL	NULL	NULL	NULL	71.6 + / -1.3 %	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DSZ cells grown in liquid medium with SZ ( in 10 mM ethanol ) as carbon source mineralized 71.6 + / -1.3 % of 0.025 mM SZ with a yield of 4.6 + / -0.3 microg cell dry weight mmol ( -1 ) carbon .
	manualset3
258562	8	426025	7	NULL	NULL	NULL	NULL	0.025 mM	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DSZ cells grown in liquid medium with SZ ( in 10 mM ethanol ) as carbon source mineralized 71.6 + / -1.3 % of 0.025 mM SZ with a yield of 4.6 + / -0.3 microg cell dry weight mmol ( -1 ) carbon .
	manualset3
258563	9	426025	7	NULL	NULL	NULL	NULL	SZ 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DSZ cells grown in liquid medium with SZ ( in 10 mM ethanol ) as carbon source mineralized 71.6 + / -1.3 % of 0.025 mM SZ with a yield of 4.6 + / -0.3 microg cell dry weight mmol ( -1 ) carbon .
	manualset3
258564	10	426025	7	NULL	NULL	NULL	NULL	yield	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DSZ cells grown in liquid medium with SZ ( in 10 mM ethanol ) as carbon source mineralized 71.6 + / -1.3 % of 0.025 mM SZ with a yield of 4.6 + / -0.3 microg cell dry weight mmol ( -1 ) carbon .
	manualset3
258565	11	426025	7	NULL	NULL	NULL	NULL	4.6 + / -0.3 microg cell dry weight mmol ( -1 ) carbon 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DSZ cells grown in liquid medium with SZ ( in 10 mM ethanol ) as carbon source mineralized 71.6 + / -1.3 % of 0.025 mM SZ with a yield of 4.6 + / -0.3 microg cell dry weight mmol ( -1 ) carbon .
	manualset3
258567	1	426026	7	NULL	NULL	NULL	NULL	DUE programs	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DUE programs were developed at Western Missouri Mental Health Center to monitor prescribing of medications in the hospital and ambulatory-care settings .
	manualset3
258568	2	426026	7	NULL	NULL	NULL	NULL	Western Missouri Mental Health Center	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DUE programs were developed at Western Missouri Mental Health Center to monitor prescribing of medications in the hospital and ambulatory-care settings .
	manualset3
258569	3	426026	7	NULL	NULL	NULL	NULL	medications	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DUE programs were developed at Western Missouri Mental Health Center to monitor prescribing of medications in the hospital and ambulatory-care settings .
	manualset3
258570	4	426026	7	NULL	NULL	NULL	NULL	hospital	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DUE programs were developed at Western Missouri Mental Health Center to monitor prescribing of medications in the hospital and ambulatory-care settings .
	manualset3
258571	5	426026	7	NULL	NULL	NULL	NULL	ambulatory-care settings	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DUE programs were developed at Western Missouri Mental Health Center to monitor prescribing of medications in the hospital and ambulatory-care settings .
	manualset3
258572	1	426027	7	NULL	NULL	NULL	NULL	Dacron bags 	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dacron bags containing these fractions were incubated in the rumen of a steer and the residue that remained was analyzed sequentially for DM , NDF , ADF , ADL , and acid detergent insoluble ash .
	manualset3
258573	2	426027	7	NULL	NULL	NULL	NULL	fractions 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dacron bags containing these fractions were incubated in the rumen of a steer and the residue that remained was analyzed sequentially for DM , NDF , ADF , ADL , and acid detergent insoluble ash .
	manualset3
258574	3	426027	7	NULL	NULL	NULL	NULL	rumen 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dacron bags containing these fractions were incubated in the rumen of a steer and the residue that remained was analyzed sequentially for DM , NDF , ADF , ADL , and acid detergent insoluble ash .
	manualset3
258575	4	426027	7	NULL	NULL	NULL	NULL	 steer	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dacron bags containing these fractions were incubated in the rumen of a steer and the residue that remained was analyzed sequentially for DM , NDF , ADF , ADL , and acid detergent insoluble ash .
	manualset3
258576	5	426027	7	NULL	NULL	NULL	NULL	residue	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dacron bags containing these fractions were incubated in the rumen of a steer and the residue that remained was analyzed sequentially for DM , NDF , ADF , ADL , and acid detergent insoluble ash .
	manualset3
258577	6	426027	7	NULL	NULL	NULL	NULL	DM	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dacron bags containing these fractions were incubated in the rumen of a steer and the residue that remained was analyzed sequentially for DM , NDF , ADF , ADL , and acid detergent insoluble ash .
	manualset3
258578	7	426027	7	NULL	NULL	NULL	NULL	NDF	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dacron bags containing these fractions were incubated in the rumen of a steer and the residue that remained was analyzed sequentially for DM , NDF , ADF , ADL , and acid detergent insoluble ash .
	manualset3
258579	8	426027	7	NULL	NULL	NULL	NULL	ADF	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dacron bags containing these fractions were incubated in the rumen of a steer and the residue that remained was analyzed sequentially for DM , NDF , ADF , ADL , and acid detergent insoluble ash .
	manualset3
258580	9	426027	7	NULL	NULL	NULL	NULL	ADL	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dacron bags containing these fractions were incubated in the rumen of a steer and the residue that remained was analyzed sequentially for DM , NDF , ADF , ADL , and acid detergent insoluble ash .
	manualset3
258581	10	426027	7	NULL	NULL	NULL	NULL	acid detergent insoluble ash	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dacron bags containing these fractions were incubated in the rumen of a steer and the residue that remained was analyzed sequentially for DM , NDF , ADF , ADL , and acid detergent insoluble ash .
	manualset3
258582	1	426028	7	NULL	NULL	NULL	NULL	Dahl salt-resistant rats ( R rats )	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dahl salt-resistant rats ( R rats ) on either 8 % or 0.11 % NaCl had normal BP .
	manualset3
258583	2	426028	7	NULL	NULL	NULL	NULL	 8 %	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dahl salt-resistant rats ( R rats ) on either 8 % or 0.11 % NaCl had normal BP .
	manualset3
258584	3	426028	7	NULL	NULL	NULL	NULL	0.11 %	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dahl salt-resistant rats ( R rats ) on either 8 % or 0.11 % NaCl had normal BP .
	manualset3
258585	4	426028	7	NULL	NULL	NULL	NULL	NaCl 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dahl salt-resistant rats ( R rats ) on either 8 % or 0.11 % NaCl had normal BP .
	manualset3
258586	5	426028	7	NULL	NULL	NULL	NULL	normal BP	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dahl salt-resistant rats ( R rats ) on either 8 % or 0.11 % NaCl had normal BP .
	manualset3
258587	1	426029	7	NULL	NULL	NULL	NULL	Daily administration	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Daily administration of IL-2 ( 50 x 10 ( 5 ) U ) was started 3 days prior to the first LAK infusion and continued throughout the cycle .
	manualset3
258588	2	426029	7	NULL	NULL	NULL	NULL	 IL-2	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Daily administration of IL-2 ( 50 x 10 ( 5 ) U ) was started 3 days prior to the first LAK infusion and continued throughout the cycle .
	manualset3
258589	3	426029	7	NULL	NULL	NULL	NULL	( 50 x 10 ( 5 ) U )	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Daily administration of IL-2 ( 50 x 10 ( 5 ) U ) was started 3 days prior to the first LAK infusion and continued throughout the cycle .
	manualset3
258590	4	426029	7	NULL	NULL	NULL	NULL	 3 days	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Daily administration of IL-2 ( 50 x 10 ( 5 ) U ) was started 3 days prior to the first LAK infusion and continued throughout the cycle .
	manualset3
258591	5	426029	7	NULL	NULL	NULL	NULL	first LAK infusion 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Daily administration of IL-2 ( 50 x 10 ( 5 ) U ) was started 3 days prior to the first LAK infusion and continued throughout the cycle .
	manualset3
258592	6	426029	7	NULL	NULL	NULL	NULL	cycle	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Daily administration of IL-2 ( 50 x 10 ( 5 ) U ) was started 3 days prior to the first LAK infusion and continued throughout the cycle .
	manualset3
258593	1	426030	7	NULL	NULL	NULL	NULL	Molecular diagnosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Molecular diagnosis of fragile X-chromosome syndrome ( Martin-Bell syndrome ) in patients of native populations ) .
	manualset3
258594	2	426030	7	NULL	NULL	NULL	NULL	 fragile X-chromosome syndrome ( Martin-Bell syndrome ) 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Molecular diagnosis of fragile X-chromosome syndrome ( Martin-Bell syndrome ) in patients of native populations ) .
	manualset3
258595	3	426030	7	NULL	NULL	NULL	NULL	 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Molecular diagnosis of fragile X-chromosome syndrome ( Martin-Bell syndrome ) in patients of native populations ) .
	manualset3
258596	4	426030	7	NULL	NULL	NULL	NULL	native populations	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Molecular diagnosis of fragile X-chromosome syndrome ( Martin-Bell syndrome ) in patients of native populations ) .
	manualset3
258971	1	426031	7	NULL	NULL	NULL	NULL	Daphnia lumholtzi G. O. Sars	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Daphnia lumholtzi G. O. Sars , 1885 , a native cladoceran from Australia , Southwestern Asia and North Africa , has recently been found in the Neotropical region .
	manualset3
258972	2	426031	7	NULL	NULL	NULL	NULL	 1885 	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Daphnia lumholtzi G. O. Sars , 1885 , a native cladoceran from Australia , Southwestern Asia and North Africa , has recently been found in the Neotropical region .
	manualset3
258973	3	426031	7	NULL	NULL	NULL	NULL	native cladoceran	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Daphnia lumholtzi G. O. Sars , 1885 , a native cladoceran from Australia , Southwestern Asia and North Africa , has recently been found in the Neotropical region .
	manualset3
258974	4	426031	7	NULL	NULL	NULL	NULL	Australia	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Daphnia lumholtzi G. O. Sars , 1885 , a native cladoceran from Australia , Southwestern Asia and North Africa , has recently been found in the Neotropical region .
	manualset3
258975	5	426031	7	NULL	NULL	NULL	NULL	Southwestern Asia	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Daphnia lumholtzi G. O. Sars , 1885 , a native cladoceran from Australia , Southwestern Asia and North Africa , has recently been found in the Neotropical region .
	manualset3
258976	6	426031	7	NULL	NULL	NULL	NULL	North Africa	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Daphnia lumholtzi G. O. Sars , 1885 , a native cladoceran from Australia , Southwestern Asia and North Africa , has recently been found in the Neotropical region .
	manualset3
258977	7	426031	7	NULL	NULL	NULL	NULL	Neotropical region	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Daphnia lumholtzi G. O. Sars , 1885 , a native cladoceran from Australia , Southwestern Asia and North Africa , has recently been found in the Neotropical region .
	manualset3
258978	1	426032	7	NULL	NULL	NULL	NULL	Dapsone	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dapsone in the management of `` insect bite-like reaction '' in a patient with chronic lymphocytic leukemia .
	manualset3
258979	2	426032	7	NULL	NULL	NULL	NULL	management 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dapsone in the management of `` insect bite-like reaction '' in a patient with chronic lymphocytic leukemia .
	manualset3
258980	3	426032	7	NULL	NULL	NULL	NULL	 `` insect bite-like reaction '' 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dapsone in the management of `` insect bite-like reaction '' in a patient with chronic lymphocytic leukemia .
	manualset3
258981	4	426032	7	NULL	NULL	NULL	NULL	 patient 	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dapsone in the management of `` insect bite-like reaction '' in a patient with chronic lymphocytic leukemia .
	manualset3
258982	5	426032	7	NULL	NULL	NULL	NULL	 chronic lymphocytic leukemia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dapsone in the management of `` insect bite-like reaction '' in a patient with chronic lymphocytic leukemia .
	manualset3
258983	1	426033	7	NULL	NULL	NULL	NULL	Dark resetting 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dark resetting was blocked by pre-treatment with a 5-HT ( 7 ) antagonist , but not with a 5-HT ( 1A ) antagonist .
	manualset3
258984	2	426033	7	NULL	NULL	NULL	NULL	 pre-treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dark resetting was blocked by pre-treatment with a 5-HT ( 7 ) antagonist , but not with a 5-HT ( 1A ) antagonist .
	manualset3
258985	3	426033	7	NULL	NULL	NULL	NULL	 5-HT ( 7 ) antagonist	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dark resetting was blocked by pre-treatment with a 5-HT ( 7 ) antagonist , but not with a 5-HT ( 1A ) antagonist .
	manualset3
258986	4	426033	7	NULL	NULL	NULL	NULL	5-HT ( 1A ) antagonist 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dark resetting was blocked by pre-treatment with a 5-HT ( 7 ) antagonist , but not with a 5-HT ( 1A ) antagonist .
	manualset3
258987	1	426034	7	NULL	NULL	NULL	NULL	Data collection methods	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data collection methods for analyzing the quality of the dispensing in pharmacies .
	manualset3
258988	2	426034	7	NULL	NULL	NULL	NULL	quality	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data collection methods for analyzing the quality of the dispensing in pharmacies .
	manualset3
258989	3	426034	7	NULL	NULL	NULL	NULL	dispensing	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data collection methods for analyzing the quality of the dispensing in pharmacies .
	manualset3
258990	4	426034	7	NULL	NULL	NULL	NULL	pharmacies	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data collection methods for analyzing the quality of the dispensing in pharmacies .
	manualset3
258998	1	426035	7	NULL	NULL	NULL	NULL	Data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data accumulated from in vitro and animal studies suggest that glimepiride has the least cardiotoxic potential .
	manualset3
258999	2	426035	7	NULL	NULL	NULL	NULL	 in vitro studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data accumulated from in vitro and animal studies suggest that glimepiride has the least cardiotoxic potential .
	manualset3
259000	3	426035	7	NULL	NULL	NULL	NULL	animal studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data accumulated from in vitro and animal studies suggest that glimepiride has the least cardiotoxic potential .
	manualset3
259001	4	426035	7	NULL	NULL	NULL	NULL	glimepiride	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data accumulated from in vitro and animal studies suggest that glimepiride has the least cardiotoxic potential .
	manualset3
259002	5	426035	7	NULL	NULL	NULL	NULL	cardiotoxic potential	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data accumulated from in vitro and animal studies suggest that glimepiride has the least cardiotoxic potential .
	manualset3
259003	1	426036	7	NULL	NULL	NULL	NULL	Data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data are presented on antimicrobial resistance among isolates of Streptococcus pneumoniae , Streptoco-ccus pyogenes , Haemophilus influenzae , and Moraxella catarrhalis collected in Japan during years 1-3 ( 1999-2002 ) of the Prospective Resistant Organism Tracking and Epidemiology for the Ketolide Telithromycin ( PROTEKT ) surveillance study .
	manualset3
259004	2	426036	7	NULL	NULL	NULL	NULL	antimicrobial resistance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data are presented on antimicrobial resistance among isolates of Streptococcus pneumoniae , Streptoco-ccus pyogenes , Haemophilus influenzae , and Moraxella catarrhalis collected in Japan during years 1-3 ( 1999-2002 ) of the Prospective Resistant Organism Tracking and Epidemiology for the Ketolide Telithromycin ( PROTEKT ) surveillance study .
	manualset3
259005	3	426036	7	NULL	NULL	NULL	NULL	 isolates 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data are presented on antimicrobial resistance among isolates of Streptococcus pneumoniae , Streptoco-ccus pyogenes , Haemophilus influenzae , and Moraxella catarrhalis collected in Japan during years 1-3 ( 1999-2002 ) of the Prospective Resistant Organism Tracking and Epidemiology for the Ketolide Telithromycin ( PROTEKT ) surveillance study .
	manualset3
259006	4	426036	7	NULL	NULL	NULL	NULL	Streptococcus pneumoniae	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data are presented on antimicrobial resistance among isolates of Streptococcus pneumoniae , Streptoco-ccus pyogenes , Haemophilus influenzae , and Moraxella catarrhalis collected in Japan during years 1-3 ( 1999-2002 ) of the Prospective Resistant Organism Tracking and Epidemiology for the Ketolide Telithromycin ( PROTEKT ) surveillance study .
	manualset3
259007	5	426036	7	NULL	NULL	NULL	NULL	Haemophilus influenzae	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data are presented on antimicrobial resistance among isolates of Streptococcus pneumoniae , Streptoco-ccus pyogenes , Haemophilus influenzae , and Moraxella catarrhalis collected in Japan during years 1-3 ( 1999-2002 ) of the Prospective Resistant Organism Tracking and Epidemiology for the Ketolide Telithromycin ( PROTEKT ) surveillance study .
	manualset3
259008	6	426036	7	NULL	NULL	NULL	NULL	Moraxella catarrhalis	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data are presented on antimicrobial resistance among isolates of Streptococcus pneumoniae , Streptoco-ccus pyogenes , Haemophilus influenzae , and Moraxella catarrhalis collected in Japan during years 1-3 ( 1999-2002 ) of the Prospective Resistant Organism Tracking and Epidemiology for the Ketolide Telithromycin ( PROTEKT ) surveillance study .
	manualset3
259009	7	426036	7	NULL	NULL	NULL	NULL	Japan	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data are presented on antimicrobial resistance among isolates of Streptococcus pneumoniae , Streptoco-ccus pyogenes , Haemophilus influenzae , and Moraxella catarrhalis collected in Japan during years 1-3 ( 1999-2002 ) of the Prospective Resistant Organism Tracking and Epidemiology for the Ketolide Telithromycin ( PROTEKT ) surveillance study .
	manualset3
259010	8	426036	7	NULL	NULL	NULL	NULL	years 1-3	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data are presented on antimicrobial resistance among isolates of Streptococcus pneumoniae , Streptoco-ccus pyogenes , Haemophilus influenzae , and Moraxella catarrhalis collected in Japan during years 1-3 ( 1999-2002 ) of the Prospective Resistant Organism Tracking and Epidemiology for the Ketolide Telithromycin ( PROTEKT ) surveillance study .
	manualset3
259011	9	426036	7	NULL	NULL	NULL	NULL	1999-2002	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data are presented on antimicrobial resistance among isolates of Streptococcus pneumoniae , Streptoco-ccus pyogenes , Haemophilus influenzae , and Moraxella catarrhalis collected in Japan during years 1-3 ( 1999-2002 ) of the Prospective Resistant Organism Tracking and Epidemiology for the Ketolide Telithromycin ( PROTEKT ) surveillance study .
	manualset3
259012	10	426036	7	NULL	NULL	NULL	NULL	Prospective Resistant Organism Tracking and Epidemiology 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data are presented on antimicrobial resistance among isolates of Streptococcus pneumoniae , Streptoco-ccus pyogenes , Haemophilus influenzae , and Moraxella catarrhalis collected in Japan during years 1-3 ( 1999-2002 ) of the Prospective Resistant Organism Tracking and Epidemiology for the Ketolide Telithromycin ( PROTEKT ) surveillance study .
	manualset3
259013	11	426036	7	NULL	NULL	NULL	NULL	Ketolide Telithromycin ( PROTEKT ) surveillance study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data are presented on antimicrobial resistance among isolates of Streptococcus pneumoniae , Streptoco-ccus pyogenes , Haemophilus influenzae , and Moraxella catarrhalis collected in Japan during years 1-3 ( 1999-2002 ) of the Prospective Resistant Organism Tracking and Epidemiology for the Ketolide Telithromycin ( PROTEKT ) surveillance study .
	manualset3
259014	12	426036	7	NULL	NULL	NULL	NULL	Streptoco-ccus pyogenes	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data are presented on antimicrobial resistance among isolates of Streptococcus pneumoniae , Streptoco-ccus pyogenes , Haemophilus influenzae , and Moraxella catarrhalis collected in Japan during years 1-3 ( 1999-2002 ) of the Prospective Resistant Organism Tracking and Epidemiology for the Ketolide Telithromycin ( PROTEKT ) surveillance study .
	manualset3
259015	1	426037	7	NULL	NULL	NULL	NULL	Data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data are presented that show a close correlation between the number of CD34 + cells mobilized into the peripheral blood ( PB ) and the number of CD34 + cells subsequently collected by leukapheresis ( R = 0.904 ) .
	manualset3
259016	2	426037	7	NULL	NULL	NULL	NULL	close correlation	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data are presented that show a close correlation between the number of CD34 + cells mobilized into the peripheral blood ( PB ) and the number of CD34 + cells subsequently collected by leukapheresis ( R = 0.904 ) .
	manualset3
259017	3	426037	7	NULL	NULL	NULL	NULL	number	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data are presented that show a close correlation between the number of CD34 + cells mobilized into the peripheral blood ( PB ) and the number of CD34 + cells subsequently collected by leukapheresis ( R = 0.904 ) .
	manualset3
259018	4	426037	7	NULL	NULL	NULL	NULL	CD34 + cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data are presented that show a close correlation between the number of CD34 + cells mobilized into the peripheral blood ( PB ) and the number of CD34 + cells subsequently collected by leukapheresis ( R = 0.904 ) .
	manualset3
259019	5	426037	7	NULL	NULL	NULL	NULL	peripheral blood ( PB )	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data are presented that show a close correlation between the number of CD34 + cells mobilized into the peripheral blood ( PB ) and the number of CD34 + cells subsequently collected by leukapheresis ( R = 0.904 ) .
	manualset3
259020	6	426037	7	NULL	NULL	NULL	NULL	number	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data are presented that show a close correlation between the number of CD34 + cells mobilized into the peripheral blood ( PB ) and the number of CD34 + cells subsequently collected by leukapheresis ( R = 0.904 ) .
	manualset3
259021	7	426037	7	NULL	NULL	NULL	NULL	CD34 + cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data are presented that show a close correlation between the number of CD34 + cells mobilized into the peripheral blood ( PB ) and the number of CD34 + cells subsequently collected by leukapheresis ( R = 0.904 ) .
	manualset3
259022	8	426037	7	NULL	NULL	NULL	NULL	leukapheresis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data are presented that show a close correlation between the number of CD34 + cells mobilized into the peripheral blood ( PB ) and the number of CD34 + cells subsequently collected by leukapheresis ( R = 0.904 ) .
	manualset3
259023	9	426037	7	NULL	NULL	NULL	NULL	R = 0.904	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data are presented that show a close correlation between the number of CD34 + cells mobilized into the peripheral blood ( PB ) and the number of CD34 + cells subsequently collected by leukapheresis ( R = 0.904 ) .
	manualset3
259024	1	426038	7	NULL	NULL	NULL	NULL	Data extraction	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data extraction and analyses and quality assessment were conducted according to the Cochrane standards .
	manualset3
259025	2	426038	7	NULL	NULL	NULL	NULL	analyses	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data extraction and analyses and quality assessment were conducted according to the Cochrane standards .
	manualset3
259026	3	426038	7	NULL	NULL	NULL	NULL	quality assessment	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data extraction and analyses and quality assessment were conducted according to the Cochrane standards .
	manualset3
259027	4	426038	7	NULL	NULL	NULL	NULL	Cochrane standards	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data extraction and analyses and quality assessment were conducted according to the Cochrane standards .
	manualset3
259028	1	426039	7	NULL	NULL	NULL	NULL	Data 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from an open-label , randomized , three-way crossover study in patients with perennial allergic rhinitis receiving three doses ( 100 , 200 , and 400 microg ) of a nasal solution-based triamcinolone acetonide formulation ( Tri-Nasal ) over 7 days were used to describe the pharmacokinetics of this formulation .
	manualset3
259029	2	426039	7	NULL	NULL	NULL	NULL	three-way crossover study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from an open-label , randomized , three-way crossover study in patients with perennial allergic rhinitis receiving three doses ( 100 , 200 , and 400 microg ) of a nasal solution-based triamcinolone acetonide formulation ( Tri-Nasal ) over 7 days were used to describe the pharmacokinetics of this formulation .
	manualset3
259030	3	426039	7	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from an open-label , randomized , three-way crossover study in patients with perennial allergic rhinitis receiving three doses ( 100 , 200 , and 400 microg ) of a nasal solution-based triamcinolone acetonide formulation ( Tri-Nasal ) over 7 days were used to describe the pharmacokinetics of this formulation .
	manualset3
259031	4	426039	7	NULL	NULL	NULL	NULL	perennial allergic rhinitis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from an open-label , randomized , three-way crossover study in patients with perennial allergic rhinitis receiving three doses ( 100 , 200 , and 400 microg ) of a nasal solution-based triamcinolone acetonide formulation ( Tri-Nasal ) over 7 days were used to describe the pharmacokinetics of this formulation .
	manualset3
259032	5	426039	7	NULL	NULL	NULL	NULL	three doses 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from an open-label , randomized , three-way crossover study in patients with perennial allergic rhinitis receiving three doses ( 100 , 200 , and 400 microg ) of a nasal solution-based triamcinolone acetonide formulation ( Tri-Nasal ) over 7 days were used to describe the pharmacokinetics of this formulation .
	manualset3
259033	6	426039	7	NULL	NULL	NULL	NULL	100 microg	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from an open-label , randomized , three-way crossover study in patients with perennial allergic rhinitis receiving three doses ( 100 , 200 , and 400 microg ) of a nasal solution-based triamcinolone acetonide formulation ( Tri-Nasal ) over 7 days were used to describe the pharmacokinetics of this formulation .
	manualset3
259034	7	426039	7	NULL	NULL	NULL	NULL	200  microg	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from an open-label , randomized , three-way crossover study in patients with perennial allergic rhinitis receiving three doses ( 100 , 200 , and 400 microg ) of a nasal solution-based triamcinolone acetonide formulation ( Tri-Nasal ) over 7 days were used to describe the pharmacokinetics of this formulation .
	manualset3
259035	8	426039	7	NULL	NULL	NULL	NULL	400 microg	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from an open-label , randomized , three-way crossover study in patients with perennial allergic rhinitis receiving three doses ( 100 , 200 , and 400 microg ) of a nasal solution-based triamcinolone acetonide formulation ( Tri-Nasal ) over 7 days were used to describe the pharmacokinetics of this formulation .
	manualset3
259036	9	426039	7	NULL	NULL	NULL	NULL	 nasal solution-based triamcinolone acetonide formulation ( Tri-Nasal )	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from an open-label , randomized , three-way crossover study in patients with perennial allergic rhinitis receiving three doses ( 100 , 200 , and 400 microg ) of a nasal solution-based triamcinolone acetonide formulation ( Tri-Nasal ) over 7 days were used to describe the pharmacokinetics of this formulation .
	manualset3
259037	10	426039	7	NULL	NULL	NULL	NULL	7 days	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from an open-label , randomized , three-way crossover study in patients with perennial allergic rhinitis receiving three doses ( 100 , 200 , and 400 microg ) of a nasal solution-based triamcinolone acetonide formulation ( Tri-Nasal ) over 7 days were used to describe the pharmacokinetics of this formulation .
	manualset3
259038	11	426039	7	NULL	NULL	NULL	NULL	pharmacokinetics	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from an open-label , randomized , three-way crossover study in patients with perennial allergic rhinitis receiving three doses ( 100 , 200 , and 400 microg ) of a nasal solution-based triamcinolone acetonide formulation ( Tri-Nasal ) over 7 days were used to describe the pharmacokinetics of this formulation .
	manualset3
259039	12	426039	7	NULL	NULL	NULL	NULL	 formulation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from an open-label , randomized , three-way crossover study in patients with perennial allergic rhinitis receiving three doses ( 100 , 200 , and 400 microg ) of a nasal solution-based triamcinolone acetonide formulation ( Tri-Nasal ) over 7 days were used to describe the pharmacokinetics of this formulation .
	manualset3
262791	13	426039	7	NULL	NULL	NULL	NULL	 open-label	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from an open-label , randomized , three-way crossover study in patients with perennial allergic rhinitis receiving three doses ( 100 , 200 , and 400 microg ) of a nasal solution-based triamcinolone acetonide formulation ( Tri-Nasal ) over 7 days were used to describe the pharmacokinetics of this formulation .
	manualset3
259040	1	426040	7	NULL	NULL	NULL	NULL	Data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from tests of protective activity activity obtained during a period of 3 years with whole homogenate and F and M fraction are also presented Protective activity against lethal challenge doses of trypomastigotes is strongly associated with the flagellar fraction .
	manualset3
259041	2	426040	7	NULL	NULL	NULL	NULL	 tests	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from tests of protective activity activity obtained during a period of 3 years with whole homogenate and F and M fraction are also presented Protective activity against lethal challenge doses of trypomastigotes is strongly associated with the flagellar fraction .
	manualset3
259042	3	426040	7	NULL	NULL	NULL	NULL	protective activity activity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from tests of protective activity activity obtained during a period of 3 years with whole homogenate and F and M fraction are also presented Protective activity against lethal challenge doses of trypomastigotes is strongly associated with the flagellar fraction .
	manualset3
259043	4	426040	7	NULL	NULL	NULL	NULL	period 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from tests of protective activity activity obtained during a period of 3 years with whole homogenate and F and M fraction are also presented Protective activity against lethal challenge doses of trypomastigotes is strongly associated with the flagellar fraction .
	manualset3
259044	5	426040	7	NULL	NULL	NULL	NULL	3 years	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from tests of protective activity activity obtained during a period of 3 years with whole homogenate and F and M fraction are also presented Protective activity against lethal challenge doses of trypomastigotes is strongly associated with the flagellar fraction .
	manualset3
259045	6	426040	7	NULL	NULL	NULL	NULL	whole homogenate fraction	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from tests of protective activity activity obtained during a period of 3 years with whole homogenate and F and M fraction are also presented Protective activity against lethal challenge doses of trypomastigotes is strongly associated with the flagellar fraction .
	manualset3
259046	7	426040	7	NULL	NULL	NULL	NULL	F fraction	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from tests of protective activity activity obtained during a period of 3 years with whole homogenate and F and M fraction are also presented Protective activity against lethal challenge doses of trypomastigotes is strongly associated with the flagellar fraction .
	manualset3
259047	8	426040	7	NULL	NULL	NULL	NULL	M fraction	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from tests of protective activity activity obtained during a period of 3 years with whole homogenate and F and M fraction are also presented Protective activity against lethal challenge doses of trypomastigotes is strongly associated with the flagellar fraction .
	manualset3
259048	9	426040	7	NULL	NULL	NULL	NULL	Protective activity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from tests of protective activity activity obtained during a period of 3 years with whole homogenate and F and M fraction are also presented Protective activity against lethal challenge doses of trypomastigotes is strongly associated with the flagellar fraction .
	manualset3
259049	10	426040	7	NULL	NULL	NULL	NULL	lethal challenge doses	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from tests of protective activity activity obtained during a period of 3 years with whole homogenate and F and M fraction are also presented Protective activity against lethal challenge doses of trypomastigotes is strongly associated with the flagellar fraction .
	manualset3
259050	11	426040	7	NULL	NULL	NULL	NULL	 trypomastigotes	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from tests of protective activity activity obtained during a period of 3 years with whole homogenate and F and M fraction are also presented Protective activity against lethal challenge doses of trypomastigotes is strongly associated with the flagellar fraction .
	manualset3
259051	12	426040	7	NULL	NULL	NULL	NULL	 flagellar fraction	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from tests of protective activity activity obtained during a period of 3 years with whole homogenate and F and M fraction are also presented Protective activity against lethal challenge doses of trypomastigotes is strongly associated with the flagellar fraction .
	manualset3
259052	1	426041	7	NULL	NULL	NULL	NULL	Data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from the Third National Cancer Survey indicate that the annual incidence of retinoblastoma in the United States is 11.0 new cases per million children under the age of 5 years .
	manualset3
259053	2	426041	7	NULL	NULL	NULL	NULL	Third National Cancer Survey	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from the Third National Cancer Survey indicate that the annual incidence of retinoblastoma in the United States is 11.0 new cases per million children under the age of 5 years .
	manualset3
259054	3	426041	7	NULL	NULL	NULL	NULL	annual incidence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from the Third National Cancer Survey indicate that the annual incidence of retinoblastoma in the United States is 11.0 new cases per million children under the age of 5 years .
	manualset3
259055	4	426041	7	NULL	NULL	NULL	NULL	retinoblastoma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from the Third National Cancer Survey indicate that the annual incidence of retinoblastoma in the United States is 11.0 new cases per million children under the age of 5 years .
	manualset3
259056	5	426041	7	NULL	NULL	NULL	NULL	United States	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from the Third National Cancer Survey indicate that the annual incidence of retinoblastoma in the United States is 11.0 new cases per million children under the age of 5 years .
	manualset3
259057	6	426041	7	NULL	NULL	NULL	NULL	11.0 new cases per million children	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from the Third National Cancer Survey indicate that the annual incidence of retinoblastoma in the United States is 11.0 new cases per million children under the age of 5 years .
	manualset3
259058	7	426041	7	NULL	NULL	NULL	NULL	age	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from the Third National Cancer Survey indicate that the annual incidence of retinoblastoma in the United States is 11.0 new cases per million children under the age of 5 years .
	manualset3
259059	8	426041	7	NULL	NULL	NULL	NULL	5 years 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from the Third National Cancer Survey indicate that the annual incidence of retinoblastoma in the United States is 11.0 new cases per million children under the age of 5 years .
	manualset3
259060	1	426042	7	NULL	NULL	NULL	NULL	Moraxella ( Branhamella ) catarrhalis	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Moraxella ( Branhamella ) catarrhalis .
	manualset3
259116	1	426043	7	NULL	NULL	NULL	NULL	Data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from these studies suggest that particulates in the microlayer waters of the salt marsh influenced the observed increase in both the readily grown and the total numbers of bacteria .
	manualset3
259117	2	426043	7	NULL	NULL	NULL	NULL	studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from these studies suggest that particulates in the microlayer waters of the salt marsh influenced the observed increase in both the readily grown and the total numbers of bacteria .
	manualset3
259118	3	426043	7	NULL	NULL	NULL	NULL	microlayer waters	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from these studies suggest that particulates in the microlayer waters of the salt marsh influenced the observed increase in both the readily grown and the total numbers of bacteria .
	manualset3
259119	4	426043	7	NULL	NULL	NULL	NULL	salt marsh	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from these studies suggest that particulates in the microlayer waters of the salt marsh influenced the observed increase in both the readily grown and the total numbers of bacteria .
	manualset3
259120	5	426043	7	NULL	NULL	NULL	NULL	 total numbers	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from these studies suggest that particulates in the microlayer waters of the salt marsh influenced the observed increase in both the readily grown and the total numbers of bacteria .
	manualset3
259121	6	426043	7	NULL	NULL	NULL	NULL	bacteria	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data from these studies suggest that particulates in the microlayer waters of the salt marsh influenced the observed increase in both the readily grown and the total numbers of bacteria .
	manualset3
259122	1	426044	7	NULL	NULL	NULL	NULL	Data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data generated from four structured focus group sessions , investigator fieldnotes , and clinic records of participants yielded the following themes : ( 1 ) turning points facilitated the management experience along with certain obstacles and barriers , ( 2 ) an organizational culture of caring facilitated learning self-management , ( 3 ) major shifts in provider-patient relationships accompanied a phasic process of learning management , and ( 4 ) a set of personal characteristics most likely influenced the learning process .
	manualset3
259123	2	426044	7	NULL	NULL	NULL	NULL	four structured focus group sessions	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data generated from four structured focus group sessions , investigator fieldnotes , and clinic records of participants yielded the following themes : ( 1 ) turning points facilitated the management experience along with certain obstacles and barriers , ( 2 ) an organizational culture of caring facilitated learning self-management , ( 3 ) major shifts in provider-patient relationships accompanied a phasic process of learning management , and ( 4 ) a set of personal characteristics most likely influenced the learning process .
	manualset3
259124	3	426044	7	NULL	NULL	NULL	NULL	investigator fieldnotes	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data generated from four structured focus group sessions , investigator fieldnotes , and clinic records of participants yielded the following themes : ( 1 ) turning points facilitated the management experience along with certain obstacles and barriers , ( 2 ) an organizational culture of caring facilitated learning self-management , ( 3 ) major shifts in provider-patient relationships accompanied a phasic process of learning management , and ( 4 ) a set of personal characteristics most likely influenced the learning process .
	manualset3
259125	4	426044	7	NULL	NULL	NULL	NULL	clinic records	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data generated from four structured focus group sessions , investigator fieldnotes , and clinic records of participants yielded the following themes : ( 1 ) turning points facilitated the management experience along with certain obstacles and barriers , ( 2 ) an organizational culture of caring facilitated learning self-management , ( 3 ) major shifts in provider-patient relationships accompanied a phasic process of learning management , and ( 4 ) a set of personal characteristics most likely influenced the learning process .
	manualset3
259126	5	426044	7	NULL	NULL	NULL	NULL	participants	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data generated from four structured focus group sessions , investigator fieldnotes , and clinic records of participants yielded the following themes : ( 1 ) turning points facilitated the management experience along with certain obstacles and barriers , ( 2 ) an organizational culture of caring facilitated learning self-management , ( 3 ) major shifts in provider-patient relationships accompanied a phasic process of learning management , and ( 4 ) a set of personal characteristics most likely influenced the learning process .
	manualset3
259127	6	426044	7	NULL	NULL	NULL	NULL	following themes	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data generated from four structured focus group sessions , investigator fieldnotes , and clinic records of participants yielded the following themes : ( 1 ) turning points facilitated the management experience along with certain obstacles and barriers , ( 2 ) an organizational culture of caring facilitated learning self-management , ( 3 ) major shifts in provider-patient relationships accompanied a phasic process of learning management , and ( 4 ) a set of personal characteristics most likely influenced the learning process .
	manualset3
259128	7	426044	7	NULL	NULL	NULL	NULL	 turning points	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data generated from four structured focus group sessions , investigator fieldnotes , and clinic records of participants yielded the following themes : ( 1 ) turning points facilitated the management experience along with certain obstacles and barriers , ( 2 ) an organizational culture of caring facilitated learning self-management , ( 3 ) major shifts in provider-patient relationships accompanied a phasic process of learning management , and ( 4 ) a set of personal characteristics most likely influenced the learning process .
	manualset3
259129	8	426044	7	NULL	NULL	NULL	NULL	management experience	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data generated from four structured focus group sessions , investigator fieldnotes , and clinic records of participants yielded the following themes : ( 1 ) turning points facilitated the management experience along with certain obstacles and barriers , ( 2 ) an organizational culture of caring facilitated learning self-management , ( 3 ) major shifts in provider-patient relationships accompanied a phasic process of learning management , and ( 4 ) a set of personal characteristics most likely influenced the learning process .
	manualset3
259130	9	426044	7	NULL	NULL	NULL	NULL	obstacles 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data generated from four structured focus group sessions , investigator fieldnotes , and clinic records of participants yielded the following themes : ( 1 ) turning points facilitated the management experience along with certain obstacles and barriers , ( 2 ) an organizational culture of caring facilitated learning self-management , ( 3 ) major shifts in provider-patient relationships accompanied a phasic process of learning management , and ( 4 ) a set of personal characteristics most likely influenced the learning process .
	manualset3
259131	10	426044	7	NULL	NULL	NULL	NULL	barriers	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data generated from four structured focus group sessions , investigator fieldnotes , and clinic records of participants yielded the following themes : ( 1 ) turning points facilitated the management experience along with certain obstacles and barriers , ( 2 ) an organizational culture of caring facilitated learning self-management , ( 3 ) major shifts in provider-patient relationships accompanied a phasic process of learning management , and ( 4 ) a set of personal characteristics most likely influenced the learning process .
	manualset3
259132	11	426044	7	NULL	NULL	NULL	NULL	organizational culture	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data generated from four structured focus group sessions , investigator fieldnotes , and clinic records of participants yielded the following themes : ( 1 ) turning points facilitated the management experience along with certain obstacles and barriers , ( 2 ) an organizational culture of caring facilitated learning self-management , ( 3 ) major shifts in provider-patient relationships accompanied a phasic process of learning management , and ( 4 ) a set of personal characteristics most likely influenced the learning process .
	manualset3
259133	12	426044	7	NULL	NULL	NULL	NULL	caring facilitated learning self-management	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data generated from four structured focus group sessions , investigator fieldnotes , and clinic records of participants yielded the following themes : ( 1 ) turning points facilitated the management experience along with certain obstacles and barriers , ( 2 ) an organizational culture of caring facilitated learning self-management , ( 3 ) major shifts in provider-patient relationships accompanied a phasic process of learning management , and ( 4 ) a set of personal characteristics most likely influenced the learning process .
	manualset3
259134	13	426044	7	NULL	NULL	NULL	NULL	major shifts	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data generated from four structured focus group sessions , investigator fieldnotes , and clinic records of participants yielded the following themes : ( 1 ) turning points facilitated the management experience along with certain obstacles and barriers , ( 2 ) an organizational culture of caring facilitated learning self-management , ( 3 ) major shifts in provider-patient relationships accompanied a phasic process of learning management , and ( 4 ) a set of personal characteristics most likely influenced the learning process .
	manualset3
259135	14	426044	7	NULL	NULL	NULL	NULL	provider-patient relationships	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data generated from four structured focus group sessions , investigator fieldnotes , and clinic records of participants yielded the following themes : ( 1 ) turning points facilitated the management experience along with certain obstacles and barriers , ( 2 ) an organizational culture of caring facilitated learning self-management , ( 3 ) major shifts in provider-patient relationships accompanied a phasic process of learning management , and ( 4 ) a set of personal characteristics most likely influenced the learning process .
	manualset3
259136	15	426044	7	NULL	NULL	NULL	NULL	phasic process	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data generated from four structured focus group sessions , investigator fieldnotes , and clinic records of participants yielded the following themes : ( 1 ) turning points facilitated the management experience along with certain obstacles and barriers , ( 2 ) an organizational culture of caring facilitated learning self-management , ( 3 ) major shifts in provider-patient relationships accompanied a phasic process of learning management , and ( 4 ) a set of personal characteristics most likely influenced the learning process .
	manualset3
259137	16	426044	7	NULL	NULL	NULL	NULL	learning management	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data generated from four structured focus group sessions , investigator fieldnotes , and clinic records of participants yielded the following themes : ( 1 ) turning points facilitated the management experience along with certain obstacles and barriers , ( 2 ) an organizational culture of caring facilitated learning self-management , ( 3 ) major shifts in provider-patient relationships accompanied a phasic process of learning management , and ( 4 ) a set of personal characteristics most likely influenced the learning process .
	manualset3
259138	17	426044	7	NULL	NULL	NULL	NULL	set	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data generated from four structured focus group sessions , investigator fieldnotes , and clinic records of participants yielded the following themes : ( 1 ) turning points facilitated the management experience along with certain obstacles and barriers , ( 2 ) an organizational culture of caring facilitated learning self-management , ( 3 ) major shifts in provider-patient relationships accompanied a phasic process of learning management , and ( 4 ) a set of personal characteristics most likely influenced the learning process .
	manualset3
259139	18	426044	7	NULL	NULL	NULL	NULL	 personal characteristics 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data generated from four structured focus group sessions , investigator fieldnotes , and clinic records of participants yielded the following themes : ( 1 ) turning points facilitated the management experience along with certain obstacles and barriers , ( 2 ) an organizational culture of caring facilitated learning self-management , ( 3 ) major shifts in provider-patient relationships accompanied a phasic process of learning management , and ( 4 ) a set of personal characteristics most likely influenced the learning process .
	manualset3
259140	19	426044	7	NULL	NULL	NULL	NULL	 learning process	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data generated from four structured focus group sessions , investigator fieldnotes , and clinic records of participants yielded the following themes : ( 1 ) turning points facilitated the management experience along with certain obstacles and barriers , ( 2 ) an organizational culture of caring facilitated learning self-management , ( 3 ) major shifts in provider-patient relationships accompanied a phasic process of learning management , and ( 4 ) a set of personal characteristics most likely influenced the learning process .
	manualset3
259141	1	426045	7	NULL	NULL	NULL	NULL	Data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data indicate that the ANSRI and most of its scales are sufficiently reliable and replicable to warrant validity research .
	manualset3
259142	2	426045	7	NULL	NULL	NULL	NULL	ANSRI	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data indicate that the ANSRI and most of its scales are sufficiently reliable and replicable to warrant validity research .
	manualset3
259143	3	426045	7	NULL	NULL	NULL	NULL	scales	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data indicate that the ANSRI and most of its scales are sufficiently reliable and replicable to warrant validity research .
	manualset3
259144	4	426045	7	NULL	NULL	NULL	NULL	 validity research	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data indicate that the ANSRI and most of its scales are sufficiently reliable and replicable to warrant validity research .
	manualset3
259145	1	426046	7	NULL	NULL	NULL	NULL	Data 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data of toxicants uptake through the skin are generalized .
	manualset3
259146	2	426046	7	NULL	NULL	NULL	NULL	toxicants uptake	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data of toxicants uptake through the skin are generalized .
	manualset3
259147	3	426046	7	NULL	NULL	NULL	NULL	 skin	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data of toxicants uptake through the skin are generalized .
	manualset3
259148	1	426047	7	NULL	NULL	NULL	NULL	Data 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data on familial trends in smoking habits and unknown gestation are also presented .
	manualset3
259149	2	426047	7	NULL	NULL	NULL	NULL	 familial trends 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data on familial trends in smoking habits and unknown gestation are also presented .
	manualset3
259150	3	426047	7	NULL	NULL	NULL	NULL	smoking habits	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data on familial trends in smoking habits and unknown gestation are also presented .
	manualset3
259151	4	426047	7	NULL	NULL	NULL	NULL	 unknown gestation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data on familial trends in smoking habits and unknown gestation are also presented .
	manualset3
259152	1	426048	7	NULL	NULL	NULL	NULL	Data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data on the postfire dynamics of soil properties in the foci of Siberian moth population outbreaks are considered .
	manualset3
259153	2	426048	7	NULL	NULL	NULL	NULL	postfire dynamics	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data on the postfire dynamics of soil properties in the foci of Siberian moth population outbreaks are considered .
	manualset3
259154	3	426048	7	NULL	NULL	NULL	NULL	soil properties	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data on the postfire dynamics of soil properties in the foci of Siberian moth population outbreaks are considered .
	manualset3
259155	4	426048	7	NULL	NULL	NULL	NULL	foci	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data on the postfire dynamics of soil properties in the foci of Siberian moth population outbreaks are considered .
	manualset3
259156	5	426048	7	NULL	NULL	NULL	NULL	Siberian moth population outbreaks	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data on the postfire dynamics of soil properties in the foci of Siberian moth population outbreaks are considered .
	manualset3
259157	1	426049	7	NULL	NULL	NULL	NULL	Data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data presented show a strong correlation between location of mAb binding and the resultant activation signal delivered .
	manualset3
259158	2	426049	7	NULL	NULL	NULL	NULL	strong correlation	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data presented show a strong correlation between location of mAb binding and the resultant activation signal delivered .
	manualset3
259159	3	426049	7	NULL	NULL	NULL	NULL	location	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data presented show a strong correlation between location of mAb binding and the resultant activation signal delivered .
	manualset3
259160	4	426049	7	NULL	NULL	NULL	NULL	mAb binding	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data presented show a strong correlation between location of mAb binding and the resultant activation signal delivered .
	manualset3
259161	5	426049	7	NULL	NULL	NULL	NULL	activation signal 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data presented show a strong correlation between location of mAb binding and the resultant activation signal delivered .
	manualset3
259168	1	426050	7	NULL	NULL	NULL	NULL	Morbidity 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Morbidity and health status of students learning the profession of a printer ) .
	manualset3
259169	2	426050	7	NULL	NULL	NULL	NULL	 health status	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Morbidity and health status of students learning the profession of a printer ) .
	manualset3
259171	3	426050	7	NULL	NULL	NULL	NULL	students	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Morbidity and health status of students learning the profession of a printer ) .
	manualset3
259173	4	426050	7	NULL	NULL	NULL	NULL	 profession	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Morbidity and health status of students learning the profession of a printer ) .
	manualset3
259174	5	426050	7	NULL	NULL	NULL	NULL	printer	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Morbidity and health status of students learning the profession of a printer ) .
	manualset3
259181	1	426051	7	NULL	NULL	NULL	NULL	Data protection	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data protection and security within TANIT .
	manualset3
259182	2	426051	7	NULL	NULL	NULL	NULL	security	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data protection and security within TANIT .
	manualset3
259184	3	426051	7	NULL	NULL	NULL	NULL	TANIT	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data protection and security within TANIT .
	manualset3
259187	1	426052	7	NULL	NULL	NULL	NULL	Data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data reveal capitation 's impact on physician compensation .
	manualset3
259188	2	426052	7	NULL	NULL	NULL	NULL	capitation 's impact 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data reveal capitation 's impact on physician compensation .
	manualset3
259189	3	426052	7	NULL	NULL	NULL	NULL	physician compensation 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data reveal capitation 's impact on physician compensation .
	manualset3
259190	1	426053	7	NULL	NULL	NULL	NULL	Data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data were analyzed and compared using both tHRV analysis and enhanced HRV ( eHRV ) analysis where we used respiration to locate the frequency interval of parasympathetic activity in HRV signal .
	manualset3
259191	2	426053	7	NULL	NULL	NULL	NULL	tHRV analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data were analyzed and compared using both tHRV analysis and enhanced HRV ( eHRV ) analysis where we used respiration to locate the frequency interval of parasympathetic activity in HRV signal .
	manualset3
259192	3	426053	7	NULL	NULL	NULL	NULL	enhanced HRV ( eHRV ) analysis 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data were analyzed and compared using both tHRV analysis and enhanced HRV ( eHRV ) analysis where we used respiration to locate the frequency interval of parasympathetic activity in HRV signal .
	manualset3
259193	4	426053	7	NULL	NULL	NULL	NULL	respiration	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data were analyzed and compared using both tHRV analysis and enhanced HRV ( eHRV ) analysis where we used respiration to locate the frequency interval of parasympathetic activity in HRV signal .
	manualset3
259194	5	426053	7	NULL	NULL	NULL	NULL	frequency interval	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data were analyzed and compared using both tHRV analysis and enhanced HRV ( eHRV ) analysis where we used respiration to locate the frequency interval of parasympathetic activity in HRV signal .
	manualset3
259195	6	426053	7	NULL	NULL	NULL	NULL	 parasympathetic activity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data were analyzed and compared using both tHRV analysis and enhanced HRV ( eHRV ) analysis where we used respiration to locate the frequency interval of parasympathetic activity in HRV signal .
	manualset3
259196	7	426053	7	NULL	NULL	NULL	NULL	HRV signal 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data were analyzed and compared using both tHRV analysis and enhanced HRV ( eHRV ) analysis where we used respiration to locate the frequency interval of parasympathetic activity in HRV signal .
	manualset3
259197	1	426054	7	NULL	NULL	NULL	NULL	Data 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data were analyzed by SPSS Ver 16.0 ( Chicago , IL , USA ) and Epi-info Ver 6.00 .
	manualset3
259198	2	426054	7	NULL	NULL	NULL	NULL	SPSS Ver 16.0	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data were analyzed by SPSS Ver 16.0 ( Chicago , IL , USA ) and Epi-info Ver 6.00 .
	manualset3
259199	3	426054	7	NULL	NULL	NULL	NULL	Chicago	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data were analyzed by SPSS Ver 16.0 ( Chicago , IL , USA ) and Epi-info Ver 6.00 .
	manualset3
259200	4	426054	7	NULL	NULL	NULL	NULL	 IL	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data were analyzed by SPSS Ver 16.0 ( Chicago , IL , USA ) and Epi-info Ver 6.00 .
	manualset3
259201	5	426054	7	NULL	NULL	NULL	NULL	USA	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data were analyzed by SPSS Ver 16.0 ( Chicago , IL , USA ) and Epi-info Ver 6.00 .
	manualset3
259202	6	426054	7	NULL	NULL	NULL	NULL	Epi-info Ver 6.00	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data were analyzed by SPSS Ver 16.0 ( Chicago , IL , USA ) and Epi-info Ver 6.00 .
	manualset3
259203	1	426055	7	NULL	NULL	NULL	NULL	Data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data were analyzed using a continuous time homogeneous Markov model of the natural history of asthma .
	manualset3
259204	2	426055	7	NULL	NULL	NULL	NULL	continuous time homogeneous Markov model	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data were analyzed using a continuous time homogeneous Markov model of the natural history of asthma .
	manualset3
259205	3	426055	7	NULL	NULL	NULL	NULL	natural history 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data were analyzed using a continuous time homogeneous Markov model of the natural history of asthma .
	manualset3
259206	4	426055	7	NULL	NULL	NULL	NULL	asthma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data were analyzed using a continuous time homogeneous Markov model of the natural history of asthma .
	manualset3
259207	1	426056	7	NULL	NULL	NULL	NULL	Morphological features	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Morphological features in diagnosis of chronic liver diseases ( author 's transl ) ) .
	manualset3
259208	2	426056	7	NULL	NULL	NULL	NULL	 diagnosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Morphological features in diagnosis of chronic liver diseases ( author 's transl ) ) .
	manualset3
259209	3	426056	7	NULL	NULL	NULL	NULL	chronic liver diseases	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Morphological features in diagnosis of chronic liver diseases ( author 's transl ) ) .
	manualset3
259210	4	426056	7	NULL	NULL	NULL	NULL	author 's transl	PublicationOrCitation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Morphological features in diagnosis of chronic liver diseases ( author 's transl ) ) .
	manualset3
259211	1	426057	7	NULL	NULL	NULL	NULL	Data mining	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data mining identified a major class of common nonspecific proteolytic products corresponding to leucine aminopeptidase ( LAP ) cleavages .
	manualset3
259212	2	426057	7	NULL	NULL	NULL	NULL	major class	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data mining identified a major class of common nonspecific proteolytic products corresponding to leucine aminopeptidase ( LAP ) cleavages .
	manualset3
259213	3	426057	7	NULL	NULL	NULL	NULL	nonspecific proteolytic products	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data mining identified a major class of common nonspecific proteolytic products corresponding to leucine aminopeptidase ( LAP ) cleavages .
	manualset3
259214	4	426057	7	NULL	NULL	NULL	NULL	leucine aminopeptidase ( LAP ) cleavages	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Data mining identified a major class of common nonspecific proteolytic products corresponding to leucine aminopeptidase ( LAP ) cleavages .
	manualset3
259215	1	426058	7	NULL	NULL	NULL	NULL	Database	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Database of HIV proteinase structures .
	manualset3
259216	2	426058	7	NULL	NULL	NULL	NULL	HIV proteinase structures	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Database of HIV proteinase structures .
	manualset3
259217	1	426059	7	NULL	NULL	NULL	NULL	Day hospital	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Day and night hospital treatment : management and finances .
	manualset3
259219	2	426059	7	NULL	NULL	NULL	NULL	night hospital	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Day and night hospital treatment : management and finances .
	manualset3
259220	3	426059	7	NULL	NULL	NULL	NULL	treatment 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Day and night hospital treatment : management and finances .
	manualset3
259221	4	426059	7	NULL	NULL	NULL	NULL	management 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Day and night hospital treatment : management and finances .
	manualset3
259222	5	426059	7	NULL	NULL	NULL	NULL	finances	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Day and night hospital treatment : management and finances .
	manualset3
259223	1	426060	7	NULL	NULL	NULL	NULL	Dde I restriction fragment length polymorphism	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dde I restriction fragment length polymorphism of the alpha 2-adrenoceptor gene does not correlate with blood pressure in the F2 generation obtained from crossing stroke-prone spontaneously hypertensive rats and Wistar-Kyoto rats .
	manualset3
259224	2	426060	7	NULL	NULL	NULL	NULL	alpha 2-adrenoceptor gene	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dde I restriction fragment length polymorphism of the alpha 2-adrenoceptor gene does not correlate with blood pressure in the F2 generation obtained from crossing stroke-prone spontaneously hypertensive rats and Wistar-Kyoto rats .
	manualset3
259225	3	426060	7	NULL	NULL	NULL	NULL	blood pressure	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dde I restriction fragment length polymorphism of the alpha 2-adrenoceptor gene does not correlate with blood pressure in the F2 generation obtained from crossing stroke-prone spontaneously hypertensive rats and Wistar-Kyoto rats .
	manualset3
259226	4	426060	7	NULL	NULL	NULL	NULL	F2 generation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dde I restriction fragment length polymorphism of the alpha 2-adrenoceptor gene does not correlate with blood pressure in the F2 generation obtained from crossing stroke-prone spontaneously hypertensive rats and Wistar-Kyoto rats .
	manualset3
259227	5	426060	7	NULL	NULL	NULL	NULL	crossing stroke-prone spontaneously hypertensive rats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dde I restriction fragment length polymorphism of the alpha 2-adrenoceptor gene does not correlate with blood pressure in the F2 generation obtained from crossing stroke-prone spontaneously hypertensive rats and Wistar-Kyoto rats .
	manualset3
259228	6	426060	7	NULL	NULL	NULL	NULL	Wistar-Kyoto rats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dde I restriction fragment length polymorphism of the alpha 2-adrenoceptor gene does not correlate with blood pressure in the F2 generation obtained from crossing stroke-prone spontaneously hypertensive rats and Wistar-Kyoto rats .
	manualset3
259229	1	426061	7	NULL	NULL	NULL	NULL	De novo thymidylate synthesis activity 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	De novo thymidylate synthesis activity was diminished in mitochondria isolated from glyA CHO cells that lack SHMT2 activity , as well as mitochondria isolated from wild-type CHO cells treated with methotrexate , a DHFR inhibitor .
	manualset3
259230	2	426061	7	NULL	NULL	NULL	NULL	mitochondria	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	De novo thymidylate synthesis activity was diminished in mitochondria isolated from glyA CHO cells that lack SHMT2 activity , as well as mitochondria isolated from wild-type CHO cells treated with methotrexate , a DHFR inhibitor .
	manualset3
259231	3	426061	7	NULL	NULL	NULL	NULL	glyA CHO cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	De novo thymidylate synthesis activity was diminished in mitochondria isolated from glyA CHO cells that lack SHMT2 activity , as well as mitochondria isolated from wild-type CHO cells treated with methotrexate , a DHFR inhibitor .
	manualset3
259232	4	426061	7	NULL	NULL	NULL	NULL	SHMT2 activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	De novo thymidylate synthesis activity was diminished in mitochondria isolated from glyA CHO cells that lack SHMT2 activity , as well as mitochondria isolated from wild-type CHO cells treated with methotrexate , a DHFR inhibitor .
	manualset3
259233	5	426061	7	NULL	NULL	NULL	NULL	mitochondria	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	De novo thymidylate synthesis activity was diminished in mitochondria isolated from glyA CHO cells that lack SHMT2 activity , as well as mitochondria isolated from wild-type CHO cells treated with methotrexate , a DHFR inhibitor .
	manualset3
259234	6	426061	7	NULL	NULL	NULL	NULL	wild-type CHO cells 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	De novo thymidylate synthesis activity was diminished in mitochondria isolated from glyA CHO cells that lack SHMT2 activity , as well as mitochondria isolated from wild-type CHO cells treated with methotrexate , a DHFR inhibitor .
	manualset3
259235	7	426061	7	NULL	NULL	NULL	NULL	methotrexate	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	De novo thymidylate synthesis activity was diminished in mitochondria isolated from glyA CHO cells that lack SHMT2 activity , as well as mitochondria isolated from wild-type CHO cells treated with methotrexate , a DHFR inhibitor .
	manualset3
259236	8	426061	7	NULL	NULL	NULL	NULL	DHFR inhibitor	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	De novo thymidylate synthesis activity was diminished in mitochondria isolated from glyA CHO cells that lack SHMT2 activity , as well as mitochondria isolated from wild-type CHO cells treated with methotrexate , a DHFR inhibitor .
	manualset3
259237	1	426063	7	NULL	NULL	NULL	NULL	Deactivation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deactivation of neither aMS nor pMS sulcal cortex yielded any deficits on the form recognition tasks .
	manualset3
259238	2	426063	7	NULL	NULL	NULL	NULL	aMS sulcal cortex	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deactivation of neither aMS nor pMS sulcal cortex yielded any deficits on the form recognition tasks .
	manualset3
259239	3	426063	7	NULL	NULL	NULL	NULL	pMS sulcal cortex	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deactivation of neither aMS nor pMS sulcal cortex yielded any deficits on the form recognition tasks .
	manualset3
259240	4	426063	7	NULL	NULL	NULL	NULL	deficits	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deactivation of neither aMS nor pMS sulcal cortex yielded any deficits on the form recognition tasks .
	manualset3
259241	5	426063	7	NULL	NULL	NULL	NULL	 form recognition tasks	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deactivation of neither aMS nor pMS sulcal cortex yielded any deficits on the form recognition tasks .
	manualset3
259242	1	426064	7	NULL	NULL	NULL	NULL	Morphological findings 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Morphological findings of unusual interest in an `` angioma '' of the larynx ) .
	manualset3
259243	2	426064	7	NULL	NULL	NULL	NULL	unusual interest 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Morphological findings of unusual interest in an `` angioma '' of the larynx ) .
	manualset3
259244	3	426064	7	NULL	NULL	NULL	NULL	`` angioma '' 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Morphological findings of unusual interest in an `` angioma '' of the larynx ) .
	manualset3
259245	4	426064	7	NULL	NULL	NULL	NULL	larynx	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Morphological findings of unusual interest in an `` angioma '' of the larynx ) .
	manualset3
259246	1	426065	7	NULL	NULL	NULL	NULL	Deamination	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deamination of amino acids was significantly higher in the contents of the small intestine of chicks fed a meat meal compared to the freeze-dried raw materials , and this deamination was reduced by the addition of 50 p.p.m. penicillin to the meat meal .
	manualset3
259247	2	426065	7	NULL	NULL	NULL	NULL	amino acids	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deamination of amino acids was significantly higher in the contents of the small intestine of chicks fed a meat meal compared to the freeze-dried raw materials , and this deamination was reduced by the addition of 50 p.p.m. penicillin to the meat meal .
	manualset3
259248	3	426065	7	NULL	NULL	NULL	NULL	contents	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deamination of amino acids was significantly higher in the contents of the small intestine of chicks fed a meat meal compared to the freeze-dried raw materials , and this deamination was reduced by the addition of 50 p.p.m. penicillin to the meat meal .
	manualset3
259249	4	426065	7	NULL	NULL	NULL	NULL	 small intestine	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deamination of amino acids was significantly higher in the contents of the small intestine of chicks fed a meat meal compared to the freeze-dried raw materials , and this deamination was reduced by the addition of 50 p.p.m. penicillin to the meat meal .
	manualset3
259250	5	426065	7	NULL	NULL	NULL	NULL	chicks	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deamination of amino acids was significantly higher in the contents of the small intestine of chicks fed a meat meal compared to the freeze-dried raw materials , and this deamination was reduced by the addition of 50 p.p.m. penicillin to the meat meal .
	manualset3
259251	6	426065	7	NULL	NULL	NULL	NULL	meat meal 	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deamination of amino acids was significantly higher in the contents of the small intestine of chicks fed a meat meal compared to the freeze-dried raw materials , and this deamination was reduced by the addition of 50 p.p.m. penicillin to the meat meal .
	manualset3
259252	7	426065	7	NULL	NULL	NULL	NULL	freeze-dried raw materials	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deamination of amino acids was significantly higher in the contents of the small intestine of chicks fed a meat meal compared to the freeze-dried raw materials , and this deamination was reduced by the addition of 50 p.p.m. penicillin to the meat meal .
	manualset3
259253	8	426065	7	NULL	NULL	NULL	NULL	deamination	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deamination of amino acids was significantly higher in the contents of the small intestine of chicks fed a meat meal compared to the freeze-dried raw materials , and this deamination was reduced by the addition of 50 p.p.m. penicillin to the meat meal .
	manualset3
259254	9	426065	7	NULL	NULL	NULL	NULL	addition	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deamination of amino acids was significantly higher in the contents of the small intestine of chicks fed a meat meal compared to the freeze-dried raw materials , and this deamination was reduced by the addition of 50 p.p.m. penicillin to the meat meal .
	manualset3
259255	10	426065	7	NULL	NULL	NULL	NULL	50 p.p.m.	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deamination of amino acids was significantly higher in the contents of the small intestine of chicks fed a meat meal compared to the freeze-dried raw materials , and this deamination was reduced by the addition of 50 p.p.m. penicillin to the meat meal .
	manualset3
259256	11	426065	7	NULL	NULL	NULL	NULL	penicillin 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deamination of amino acids was significantly higher in the contents of the small intestine of chicks fed a meat meal compared to the freeze-dried raw materials , and this deamination was reduced by the addition of 50 p.p.m. penicillin to the meat meal .
	manualset3
259257	12	426065	7	NULL	NULL	NULL	NULL	meat meal	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deamination of amino acids was significantly higher in the contents of the small intestine of chicks fed a meat meal compared to the freeze-dried raw materials , and this deamination was reduced by the addition of 50 p.p.m. penicillin to the meat meal .
	manualset3
259258	1	426066	7	NULL	NULL	NULL	NULL	Death	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Death by edible mushroom : first report of Volvariella volvacea as an etiologic agent of invasive disease in a patient following double umbilical cord blood transplantation .
	manualset3
259259	2	426066	7	NULL	NULL	NULL	NULL	edible mushroom	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Death by edible mushroom : first report of Volvariella volvacea as an etiologic agent of invasive disease in a patient following double umbilical cord blood transplantation .
	manualset3
259260	3	426066	7	NULL	NULL	NULL	NULL	first report	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Death by edible mushroom : first report of Volvariella volvacea as an etiologic agent of invasive disease in a patient following double umbilical cord blood transplantation .
	manualset3
259261	4	426066	7	NULL	NULL	NULL	NULL	Volvariella volvacea 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Death by edible mushroom : first report of Volvariella volvacea as an etiologic agent of invasive disease in a patient following double umbilical cord blood transplantation .
	manualset3
259262	5	426066	7	NULL	NULL	NULL	NULL	etiologic agent 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Death by edible mushroom : first report of Volvariella volvacea as an etiologic agent of invasive disease in a patient following double umbilical cord blood transplantation .
	manualset3
259263	6	426066	7	NULL	NULL	NULL	NULL	invasive disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Death by edible mushroom : first report of Volvariella volvacea as an etiologic agent of invasive disease in a patient following double umbilical cord blood transplantation .
	manualset3
259264	7	426066	7	NULL	NULL	NULL	NULL	patient	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Death by edible mushroom : first report of Volvariella volvacea as an etiologic agent of invasive disease in a patient following double umbilical cord blood transplantation .
	manualset3
259265	8	426066	7	NULL	NULL	NULL	NULL	double umbilical cord blood transplantation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Death by edible mushroom : first report of Volvariella volvacea as an etiologic agent of invasive disease in a patient following double umbilical cord blood transplantation .
	manualset3
259266	1	426067	7	NULL	NULL	NULL	NULL	Death	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Death resulting from overzealous total parenteral nutrition : the refeeding syndrome revisited .
	manualset3
259267	2	426067	7	NULL	NULL	NULL	NULL	total parenteral nutrition	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Death resulting from overzealous total parenteral nutrition : the refeeding syndrome revisited .
	manualset3
259268	3	426067	7	NULL	NULL	NULL	NULL	refeeding syndrome	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Death resulting from overzealous total parenteral nutrition : the refeeding syndrome revisited .
	manualset3
259269	1	426068	7	NULL	NULL	NULL	NULL	Decapeptides	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decapeptides based on the C-terminus of human beta-defensin-3 were designed and evaluated to study the role of charge in defining the antimicrobial activity and selectivity of these peptides against Escherichia coli .
	manualset3
259270	2	426068	7	NULL	NULL	NULL	NULL	C-terminus	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decapeptides based on the C-terminus of human beta-defensin-3 were designed and evaluated to study the role of charge in defining the antimicrobial activity and selectivity of these peptides against Escherichia coli .
	manualset3
259271	3	426068	7	NULL	NULL	NULL	NULL	human beta-defensin-3	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decapeptides based on the C-terminus of human beta-defensin-3 were designed and evaluated to study the role of charge in defining the antimicrobial activity and selectivity of these peptides against Escherichia coli .
	manualset3
259272	4	426068	7	NULL	NULL	NULL	NULL	role 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decapeptides based on the C-terminus of human beta-defensin-3 were designed and evaluated to study the role of charge in defining the antimicrobial activity and selectivity of these peptides against Escherichia coli .
	manualset3
259273	5	426068	7	NULL	NULL	NULL	NULL	charge	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decapeptides based on the C-terminus of human beta-defensin-3 were designed and evaluated to study the role of charge in defining the antimicrobial activity and selectivity of these peptides against Escherichia coli .
	manualset3
259274	6	426068	7	NULL	NULL	NULL	NULL	antimicrobial activity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decapeptides based on the C-terminus of human beta-defensin-3 were designed and evaluated to study the role of charge in defining the antimicrobial activity and selectivity of these peptides against Escherichia coli .
	manualset3
259275	7	426068	7	NULL	NULL	NULL	NULL	selectivity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decapeptides based on the C-terminus of human beta-defensin-3 were designed and evaluated to study the role of charge in defining the antimicrobial activity and selectivity of these peptides against Escherichia coli .
	manualset3
259276	8	426068	7	NULL	NULL	NULL	NULL	peptides 	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decapeptides based on the C-terminus of human beta-defensin-3 were designed and evaluated to study the role of charge in defining the antimicrobial activity and selectivity of these peptides against Escherichia coli .
	manualset3
259277	9	426068	7	NULL	NULL	NULL	NULL	Escherichia coli 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decapeptides based on the C-terminus of human beta-defensin-3 were designed and evaluated to study the role of charge in defining the antimicrobial activity and selectivity of these peptides against Escherichia coli .
	manualset3
259278	1	426069	7	NULL	NULL	NULL	NULL	Decision-making tools 	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decision-making tools called decision aids ( DA ) are the most common application of SDM .
	manualset3
259279	2	426069	7	NULL	NULL	NULL	NULL	decision aids ( DA )	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decision-making tools called decision aids ( DA ) are the most common application of SDM .
	manualset3
259280	3	426069	7	NULL	NULL	NULL	NULL	 application	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decision-making tools called decision aids ( DA ) are the most common application of SDM .
	manualset3
259281	4	426069	7	NULL	NULL	NULL	NULL	 SDM	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decision-making tools called decision aids ( DA ) are the most common application of SDM .
	manualset3
259282	1	426070	7	NULL	NULL	NULL	NULL	treatment trial	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( A treatment trial : combination of physical training and group psychotherapy ) .
	manualset3
259283	2	426070	7	NULL	NULL	NULL	NULL	combination 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( A treatment trial : combination of physical training and group psychotherapy ) .
	manualset3
259284	3	426070	7	NULL	NULL	NULL	NULL	physical training	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( A treatment trial : combination of physical training and group psychotherapy ) .
	manualset3
259285	4	426070	7	NULL	NULL	NULL	NULL	group psychotherapy 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( A treatment trial : combination of physical training and group psychotherapy ) .
	manualset3
259286	1	426071	7	NULL	NULL	NULL	NULL	Morphological study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Morphological study of the myocardium in children and adults under normal conditions and in hypoxia ) .
	manualset3
259287	2	426071	7	NULL	NULL	NULL	NULL	myocardium	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Morphological study of the myocardium in children and adults under normal conditions and in hypoxia ) .
	manualset3
259288	3	426071	7	NULL	NULL	NULL	NULL	children	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Morphological study of the myocardium in children and adults under normal conditions and in hypoxia ) .
	manualset3
259289	4	426071	7	NULL	NULL	NULL	NULL	adults	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Morphological study of the myocardium in children and adults under normal conditions and in hypoxia ) .
	manualset3
259290	5	426071	7	NULL	NULL	NULL	NULL	normal conditions	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Morphological study of the myocardium in children and adults under normal conditions and in hypoxia ) .
	manualset3
259291	6	426071	7	NULL	NULL	NULL	NULL	hypoxia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Morphological study of the myocardium in children and adults under normal conditions and in hypoxia ) .
	manualset3
259292	1	426072	7	NULL	NULL	NULL	NULL	Decomposition	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decomposition of blue-green algal ( cyanobacterial ) blooms in lake mendota , wisconsin .
	manualset3
259293	2	426072	7	NULL	NULL	NULL	NULL	blue-green algal ( cyanobacterial ) blooms	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decomposition of blue-green algal ( cyanobacterial ) blooms in lake mendota , wisconsin .
	manualset3
259294	3	426072	7	NULL	NULL	NULL	NULL	lake mendota	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decomposition of blue-green algal ( cyanobacterial ) blooms in lake mendota , wisconsin .
	manualset3
259295	4	426072	7	NULL	NULL	NULL	NULL	wisconsin	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decomposition of blue-green algal ( cyanobacterial ) blooms in lake mendota , wisconsin .
	manualset3
259296	1	426073	7	NULL	NULL	NULL	NULL	Decompression 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decompression of the hip joint by aspiration should be done for diagnosis and for decompression of tension haemarthrosis .
	manualset3
259297	2	426073	7	NULL	NULL	NULL	NULL	hip joint	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decompression of the hip joint by aspiration should be done for diagnosis and for decompression of tension haemarthrosis .
	manualset3
259298	3	426073	7	NULL	NULL	NULL	NULL	aspiration	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decompression of the hip joint by aspiration should be done for diagnosis and for decompression of tension haemarthrosis .
	manualset3
259299	4	426073	7	NULL	NULL	NULL	NULL	diagnosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decompression of the hip joint by aspiration should be done for diagnosis and for decompression of tension haemarthrosis .
	manualset3
259300	5	426073	7	NULL	NULL	NULL	NULL	decompression	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decompression of the hip joint by aspiration should be done for diagnosis and for decompression of tension haemarthrosis .
	manualset3
259301	6	426073	7	NULL	NULL	NULL	NULL	tension haemarthrosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decompression of the hip joint by aspiration should be done for diagnosis and for decompression of tension haemarthrosis .
	manualset3
259302	1	426074	7	NULL	NULL	NULL	NULL	Deconstructing language	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deconstructing language by comparative gene expression : from neurobiology to microarray .
	manualset3
259303	2	426074	7	NULL	NULL	NULL	NULL	comparative gene expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deconstructing language by comparative gene expression : from neurobiology to microarray .
	manualset3
259304	3	426074	7	NULL	NULL	NULL	NULL	 neurobiology	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deconstructing language by comparative gene expression : from neurobiology to microarray .
	manualset3
259305	4	426074	7	NULL	NULL	NULL	NULL	microarray	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deconstructing language by comparative gene expression : from neurobiology to microarray .
	manualset3
259306	1	426075	7	NULL	NULL	NULL	NULL	Decoy receptors	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decoy receptors : a strategy to regulate inflammatory cytokines and chemokines .
	manualset3
259307	2	426075	7	NULL	NULL	NULL	NULL	strategy	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decoy receptors : a strategy to regulate inflammatory cytokines and chemokines .
	manualset3
259308	3	426075	7	NULL	NULL	NULL	NULL	 inflammatory cytokines	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decoy receptors : a strategy to regulate inflammatory cytokines and chemokines .
	manualset3
259309	4	426075	7	NULL	NULL	NULL	NULL	chemokines	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decoy receptors : a strategy to regulate inflammatory cytokines and chemokines .
	manualset3
259310	1	426076	7	NULL	NULL	NULL	NULL	Decrease	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decrease in malate dehydrogenase activities in peripheral leucocytes of type 1 diabetic dogs .
	manualset3
259311	2	426076	7	NULL	NULL	NULL	NULL	malate dehydrogenase activities	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decrease in malate dehydrogenase activities in peripheral leucocytes of type 1 diabetic dogs .
	manualset3
259312	3	426076	7	NULL	NULL	NULL	NULL	peripheral leucocytes	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decrease in malate dehydrogenase activities in peripheral leucocytes of type 1 diabetic dogs .
	manualset3
259313	4	426076	7	NULL	NULL	NULL	NULL	type 1 diabetic dogs	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decrease in malate dehydrogenase activities in peripheral leucocytes of type 1 diabetic dogs .
	manualset3
259314	1	426077	7	NULL	NULL	NULL	NULL	Decrease	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decrease in tissue weight was significant in whole brain , cerebrum and brain stem but not in cerebellum .
	manualset3
259315	2	426077	7	NULL	NULL	NULL	NULL	tissue weight	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decrease in tissue weight was significant in whole brain , cerebrum and brain stem but not in cerebellum .
	manualset3
259316	3	426077	7	NULL	NULL	NULL	NULL	whole brain	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decrease in tissue weight was significant in whole brain , cerebrum and brain stem but not in cerebellum .
	manualset3
259317	4	426077	7	NULL	NULL	NULL	NULL	 cerebrum	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decrease in tissue weight was significant in whole brain , cerebrum and brain stem but not in cerebellum .
	manualset3
259318	5	426077	7	NULL	NULL	NULL	NULL	brain stem	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decrease in tissue weight was significant in whole brain , cerebrum and brain stem but not in cerebellum .
	manualset3
259319	6	426077	7	NULL	NULL	NULL	NULL	cerebellum	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decrease in tissue weight was significant in whole brain , cerebrum and brain stem but not in cerebellum .
	manualset3
259320	1	426078	7	NULL	NULL	NULL	NULL	Decrease 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decrease in testicular weight , seminiferous tubule diameter and RNA and sialic acid levels after 4 weeks of vas injection were associated with the histological evidence for severe degeneration of spermatogenic elements .
	manualset3
259321	2	426078	7	NULL	NULL	NULL	NULL	testicular weight	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decrease in testicular weight , seminiferous tubule diameter and RNA and sialic acid levels after 4 weeks of vas injection were associated with the histological evidence for severe degeneration of spermatogenic elements .
	manualset3
259322	3	426078	7	NULL	NULL	NULL	NULL	seminiferous tubule diameter	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decrease in testicular weight , seminiferous tubule diameter and RNA and sialic acid levels after 4 weeks of vas injection were associated with the histological evidence for severe degeneration of spermatogenic elements .
	manualset3
259323	4	426078	7	NULL	NULL	NULL	NULL	RNA	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decrease in testicular weight , seminiferous tubule diameter and RNA and sialic acid levels after 4 weeks of vas injection were associated with the histological evidence for severe degeneration of spermatogenic elements .
	manualset3
259324	5	426078	7	NULL	NULL	NULL	NULL	sialic acid levels	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decrease in testicular weight , seminiferous tubule diameter and RNA and sialic acid levels after 4 weeks of vas injection were associated with the histological evidence for severe degeneration of spermatogenic elements .
	manualset3
259325	6	426078	7	NULL	NULL	NULL	NULL	4 weeks	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decrease in testicular weight , seminiferous tubule diameter and RNA and sialic acid levels after 4 weeks of vas injection were associated with the histological evidence for severe degeneration of spermatogenic elements .
	manualset3
259326	7	426078	7	NULL	NULL	NULL	NULL	vas injection	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decrease in testicular weight , seminiferous tubule diameter and RNA and sialic acid levels after 4 weeks of vas injection were associated with the histological evidence for severe degeneration of spermatogenic elements .
	manualset3
259327	8	426078	7	NULL	NULL	NULL	NULL	histological evidence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decrease in testicular weight , seminiferous tubule diameter and RNA and sialic acid levels after 4 weeks of vas injection were associated with the histological evidence for severe degeneration of spermatogenic elements .
	manualset3
259328	9	426078	7	NULL	NULL	NULL	NULL	severe degeneration	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decrease in testicular weight , seminiferous tubule diameter and RNA and sialic acid levels after 4 weeks of vas injection were associated with the histological evidence for severe degeneration of spermatogenic elements .
	manualset3
259329	10	426078	7	NULL	NULL	NULL	NULL	 spermatogenic elements	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decrease in testicular weight , seminiferous tubule diameter and RNA and sialic acid levels after 4 weeks of vas injection were associated with the histological evidence for severe degeneration of spermatogenic elements .
	manualset3
259330	1	426079	7	NULL	NULL	NULL	NULL	Decrease	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decrease in urinary excretion of ascorbic acid and histamine in rats after repeated immobilization stress .
	manualset3
259331	2	426079	7	NULL	NULL	NULL	NULL	urinary excretion	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decrease in urinary excretion of ascorbic acid and histamine in rats after repeated immobilization stress .
	manualset3
259332	3	426079	7	NULL	NULL	NULL	NULL	ascorbic acid	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decrease in urinary excretion of ascorbic acid and histamine in rats after repeated immobilization stress .
	manualset3
259333	4	426079	7	NULL	NULL	NULL	NULL	histamine	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decrease in urinary excretion of ascorbic acid and histamine in rats after repeated immobilization stress .
	manualset3
259334	5	426079	7	NULL	NULL	NULL	NULL	rats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decrease in urinary excretion of ascorbic acid and histamine in rats after repeated immobilization stress .
	manualset3
259335	6	426079	7	NULL	NULL	NULL	NULL	repeated immobilization stress	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decrease in urinary excretion of ascorbic acid and histamine in rats after repeated immobilization stress .
	manualset3
259601	1	426080	7	NULL	NULL	NULL	NULL	11beta-HSDII activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased 11beta-HSDII activity and mRNA levels in mesenteric arteries were observed in 8-week-old DS rats on a high-salt diet , indicating that 11beta-HSDII may play a significant role in salt sensitivity and hypertension .
	manualset3
259602	2	426080	7	NULL	NULL	NULL	NULL	mRNA levels	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased 11beta-HSDII activity and mRNA levels in mesenteric arteries were observed in 8-week-old DS rats on a high-salt diet , indicating that 11beta-HSDII may play a significant role in salt sensitivity and hypertension .
	manualset3
259603	3	426080	7	NULL	NULL	NULL	NULL	mesenteric arteries	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased 11beta-HSDII activity and mRNA levels in mesenteric arteries were observed in 8-week-old DS rats on a high-salt diet , indicating that 11beta-HSDII may play a significant role in salt sensitivity and hypertension .
	manualset3
259604	4	426080	7	NULL	NULL	NULL	NULL	8-week-old DS rats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased 11beta-HSDII activity and mRNA levels in mesenteric arteries were observed in 8-week-old DS rats on a high-salt diet , indicating that 11beta-HSDII may play a significant role in salt sensitivity and hypertension .
	manualset3
259605	5	426080	7	NULL	NULL	NULL	NULL	high-salt diet	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased 11beta-HSDII activity and mRNA levels in mesenteric arteries were observed in 8-week-old DS rats on a high-salt diet , indicating that 11beta-HSDII may play a significant role in salt sensitivity and hypertension .
	manualset3
259606	6	426080	7	NULL	NULL	NULL	NULL	11beta-HSDII	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased 11beta-HSDII activity and mRNA levels in mesenteric arteries were observed in 8-week-old DS rats on a high-salt diet , indicating that 11beta-HSDII may play a significant role in salt sensitivity and hypertension .
	manualset3
259607	7	426080	7	NULL	NULL	NULL	NULL	role 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased 11beta-HSDII activity and mRNA levels in mesenteric arteries were observed in 8-week-old DS rats on a high-salt diet , indicating that 11beta-HSDII may play a significant role in salt sensitivity and hypertension .
	manualset3
259608	8	426080	7	NULL	NULL	NULL	NULL	salt sensitivity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased 11beta-HSDII activity and mRNA levels in mesenteric arteries were observed in 8-week-old DS rats on a high-salt diet , indicating that 11beta-HSDII may play a significant role in salt sensitivity and hypertension .
	manualset3
259609	9	426080	7	NULL	NULL	NULL	NULL	hypertension	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased 11beta-HSDII activity and mRNA levels in mesenteric arteries were observed in 8-week-old DS rats on a high-salt diet , indicating that 11beta-HSDII may play a significant role in salt sensitivity and hypertension .
	manualset3
259610	1	426081	7	NULL	NULL	NULL	NULL	 AGD	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased AGD was a sensitive predictor of lesions in the male reproductive tract , relatively small changes in AGD were associated with a significant incidence of male reproductive malformations .
	manualset3
259611	2	426081	7	NULL	NULL	NULL	NULL	sensitive predictor	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased AGD was a sensitive predictor of lesions in the male reproductive tract , relatively small changes in AGD were associated with a significant incidence of male reproductive malformations .
	manualset3
259612	3	426081	7	NULL	NULL	NULL	NULL	lesions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased AGD was a sensitive predictor of lesions in the male reproductive tract , relatively small changes in AGD were associated with a significant incidence of male reproductive malformations .
	manualset3
259613	4	426081	7	NULL	NULL	NULL	NULL	male reproductive tract	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased AGD was a sensitive predictor of lesions in the male reproductive tract , relatively small changes in AGD were associated with a significant incidence of male reproductive malformations .
	manualset3
259614	5	426081	7	NULL	NULL	NULL	NULL	small changes	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased AGD was a sensitive predictor of lesions in the male reproductive tract , relatively small changes in AGD were associated with a significant incidence of male reproductive malformations .
	manualset3
259615	6	426081	7	NULL	NULL	NULL	NULL	AGD	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased AGD was a sensitive predictor of lesions in the male reproductive tract , relatively small changes in AGD were associated with a significant incidence of male reproductive malformations .
	manualset3
259616	7	426081	7	NULL	NULL	NULL	NULL	significant incidence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased AGD was a sensitive predictor of lesions in the male reproductive tract , relatively small changes in AGD were associated with a significant incidence of male reproductive malformations .
	manualset3
259617	8	426081	7	NULL	NULL	NULL	NULL	male reproductive malformations	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased AGD was a sensitive predictor of lesions in the male reproductive tract , relatively small changes in AGD were associated with a significant incidence of male reproductive malformations .
	manualset3
259618	1	426082	7	NULL	NULL	NULL	NULL	GSH/GSSG	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased GSH/GSSG and increased MDA concentrations were also viewed in the cortex and basal ganglia .
	manualset3
259619	2	426082	7	NULL	NULL	NULL	NULL	MDA concentrations	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased GSH/GSSG and increased MDA concentrations were also viewed in the cortex and basal ganglia .
	manualset3
259620	3	426082	7	NULL	NULL	NULL	NULL	cortex	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased GSH/GSSG and increased MDA concentrations were also viewed in the cortex and basal ganglia .
	manualset3
259621	4	426082	7	NULL	NULL	NULL	NULL	basal ganglia	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased GSH/GSSG and increased MDA concentrations were also viewed in the cortex and basal ganglia .
	manualset3
259622	1	426083	7	NULL	NULL	NULL	NULL	Decreased amounts 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased amounts of djenkolic acid in seedlings and young plants , as compared to the seed , indicate that this is likely the metabolic precursor of the volatile sulfur components .
	manualset3
259623	2	426083	7	NULL	NULL	NULL	NULL	djenkolic acid 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased amounts of djenkolic acid in seedlings and young plants , as compared to the seed , indicate that this is likely the metabolic precursor of the volatile sulfur components .
	manualset3
259624	3	426083	7	NULL	NULL	NULL	NULL	seedlings	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased amounts of djenkolic acid in seedlings and young plants , as compared to the seed , indicate that this is likely the metabolic precursor of the volatile sulfur components .
	manualset3
259625	4	426083	7	NULL	NULL	NULL	NULL	 young plants	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased amounts of djenkolic acid in seedlings and young plants , as compared to the seed , indicate that this is likely the metabolic precursor of the volatile sulfur components .
	manualset3
259626	5	426083	7	NULL	NULL	NULL	NULL	 seed	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased amounts of djenkolic acid in seedlings and young plants , as compared to the seed , indicate that this is likely the metabolic precursor of the volatile sulfur components .
	manualset3
259627	6	426083	7	NULL	NULL	NULL	NULL	metabolic precursor	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased amounts of djenkolic acid in seedlings and young plants , as compared to the seed , indicate that this is likely the metabolic precursor of the volatile sulfur components .
	manualset3
259628	7	426083	7	NULL	NULL	NULL	NULL	 volatile sulfur components	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased amounts of djenkolic acid in seedlings and young plants , as compared to the seed , indicate that this is likely the metabolic precursor of the volatile sulfur components .
	manualset3
259629	1	426084	7	NULL	NULL	NULL	NULL	de novo synthesis 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased de novo synthesis of glomerular proteoglycans in diabetes : biochemical and autoradiographic evidence .
	manualset3
259630	2	426084	7	NULL	NULL	NULL	NULL	glomerular proteoglycans	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased de novo synthesis of glomerular proteoglycans in diabetes : biochemical and autoradiographic evidence .
	manualset3
259631	3	426084	7	NULL	NULL	NULL	NULL	diabetes	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased de novo synthesis of glomerular proteoglycans in diabetes : biochemical and autoradiographic evidence .
	manualset3
259632	4	426084	7	NULL	NULL	NULL	NULL	 biochemical evidence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased de novo synthesis of glomerular proteoglycans in diabetes : biochemical and autoradiographic evidence .
	manualset3
259633	5	426084	7	NULL	NULL	NULL	NULL	autoradiographic evidence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased de novo synthesis of glomerular proteoglycans in diabetes : biochemical and autoradiographic evidence .
	manualset3
259634	1	426085	7	NULL	NULL	NULL	NULL	Decreased expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased expression ( twofold ) of a putative yehUTS operon of which yehUT encodes a putative YehU/YehT two-component system in the ompR mutant from Salmonella enterica serovar Typhi ( S. Typhi ) GIFU10007 under hypotonic growth condition was observed by qRT-PCR .
	manualset3
259635	2	426085	7	NULL	NULL	NULL	NULL	twofold 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased expression ( twofold ) of a putative yehUTS operon of which yehUT encodes a putative YehU/YehT two-component system in the ompR mutant from Salmonella enterica serovar Typhi ( S. Typhi ) GIFU10007 under hypotonic growth condition was observed by qRT-PCR .
	manualset3
259636	3	426085	7	NULL	NULL	NULL	NULL	 putative yehUTS operon	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased expression ( twofold ) of a putative yehUTS operon of which yehUT encodes a putative YehU/YehT two-component system in the ompR mutant from Salmonella enterica serovar Typhi ( S. Typhi ) GIFU10007 under hypotonic growth condition was observed by qRT-PCR .
	manualset3
259637	4	426085	7	NULL	NULL	NULL	NULL	 yehUT	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased expression ( twofold ) of a putative yehUTS operon of which yehUT encodes a putative YehU/YehT two-component system in the ompR mutant from Salmonella enterica serovar Typhi ( S. Typhi ) GIFU10007 under hypotonic growth condition was observed by qRT-PCR .
	manualset3
259638	5	426085	7	NULL	NULL	NULL	NULL	 putative YehU/YehT two-component system	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased expression ( twofold ) of a putative yehUTS operon of which yehUT encodes a putative YehU/YehT two-component system in the ompR mutant from Salmonella enterica serovar Typhi ( S. Typhi ) GIFU10007 under hypotonic growth condition was observed by qRT-PCR .
	manualset3
259639	6	426085	7	NULL	NULL	NULL	NULL	ompR mutant	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased expression ( twofold ) of a putative yehUTS operon of which yehUT encodes a putative YehU/YehT two-component system in the ompR mutant from Salmonella enterica serovar Typhi ( S. Typhi ) GIFU10007 under hypotonic growth condition was observed by qRT-PCR .
	manualset3
259640	7	426085	7	NULL	NULL	NULL	NULL	Salmonella enterica serovar Typhi ( S. Typhi ) GIFU10007 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased expression ( twofold ) of a putative yehUTS operon of which yehUT encodes a putative YehU/YehT two-component system in the ompR mutant from Salmonella enterica serovar Typhi ( S. Typhi ) GIFU10007 under hypotonic growth condition was observed by qRT-PCR .
	manualset3
259641	8	426085	7	NULL	NULL	NULL	NULL	hypotonic growth condition	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased expression ( twofold ) of a putative yehUTS operon of which yehUT encodes a putative YehU/YehT two-component system in the ompR mutant from Salmonella enterica serovar Typhi ( S. Typhi ) GIFU10007 under hypotonic growth condition was observed by qRT-PCR .
	manualset3
259642	9	426085	7	NULL	NULL	NULL	NULL	qRT-PCR	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased expression ( twofold ) of a putative yehUTS operon of which yehUT encodes a putative YehU/YehT two-component system in the ompR mutant from Salmonella enterica serovar Typhi ( S. Typhi ) GIFU10007 under hypotonic growth condition was observed by qRT-PCR .
	manualset3
259643	1	426086	7	NULL	NULL	NULL	NULL	Decreased expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased expression of VEGF may be a contributing factor , but the situation may be more complicated for mature retinal vessels than it is for immature vessels , because VEGF replacement does not rescue mature retinal vessels , suggesting that other factors may also be involved .
	manualset3
259644	2	426086	7	NULL	NULL	NULL	NULL	VEGF	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased expression of VEGF may be a contributing factor , but the situation may be more complicated for mature retinal vessels than it is for immature vessels , because VEGF replacement does not rescue mature retinal vessels , suggesting that other factors may also be involved .
	manualset3
259645	3	426086	7	NULL	NULL	NULL	NULL	contributing factor	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased expression of VEGF may be a contributing factor , but the situation may be more complicated for mature retinal vessels than it is for immature vessels , because VEGF replacement does not rescue mature retinal vessels , suggesting that other factors may also be involved .
	manualset3
259646	4	426086	7	NULL	NULL	NULL	NULL	 situation 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased expression of VEGF may be a contributing factor , but the situation may be more complicated for mature retinal vessels than it is for immature vessels , because VEGF replacement does not rescue mature retinal vessels , suggesting that other factors may also be involved .
	manualset3
259647	5	426086	7	NULL	NULL	NULL	NULL	mature retinal vessels	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased expression of VEGF may be a contributing factor , but the situation may be more complicated for mature retinal vessels than it is for immature vessels , because VEGF replacement does not rescue mature retinal vessels , suggesting that other factors may also be involved .
	manualset3
259648	6	426086	7	NULL	NULL	NULL	NULL	 immature vessels	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased expression of VEGF may be a contributing factor , but the situation may be more complicated for mature retinal vessels than it is for immature vessels , because VEGF replacement does not rescue mature retinal vessels , suggesting that other factors may also be involved .
	manualset3
259649	7	426086	7	NULL	NULL	NULL	NULL	VEGF replacement 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased expression of VEGF may be a contributing factor , but the situation may be more complicated for mature retinal vessels than it is for immature vessels , because VEGF replacement does not rescue mature retinal vessels , suggesting that other factors may also be involved .
	manualset3
259650	8	426086	7	NULL	NULL	NULL	NULL	mature retinal vessels	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased expression of VEGF may be a contributing factor , but the situation may be more complicated for mature retinal vessels than it is for immature vessels , because VEGF replacement does not rescue mature retinal vessels , suggesting that other factors may also be involved .
	manualset3
259651	9	426086	7	NULL	NULL	NULL	NULL	other factors	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased expression of VEGF may be a contributing factor , but the situation may be more complicated for mature retinal vessels than it is for immature vessels , because VEGF replacement does not rescue mature retinal vessels , suggesting that other factors may also be involved .
	manualset3
259652	1	426087	7	NULL	NULL	NULL	NULL	Decreased heart stroke volume	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased heart stroke volume and blood flow velocity in pulmonary circulation were found in the patients with left bundle block .
	manualset3
259653	2	426087	7	NULL	NULL	NULL	NULL	blood flow velocity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased heart stroke volume and blood flow velocity in pulmonary circulation were found in the patients with left bundle block .
	manualset3
259654	3	426087	7	NULL	NULL	NULL	NULL	pulmonary circulation 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased heart stroke volume and blood flow velocity in pulmonary circulation were found in the patients with left bundle block .
	manualset3
259655	4	426087	7	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased heart stroke volume and blood flow velocity in pulmonary circulation were found in the patients with left bundle block .
	manualset3
259656	5	426087	7	NULL	NULL	NULL	NULL	left bundle block	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased heart stroke volume and blood flow velocity in pulmonary circulation were found in the patients with left bundle block .
	manualset3
259657	1	426088	7	NULL	NULL	NULL	NULL	Decreased penetrance	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased penetrance was prominent in family members .
	manualset3
259658	2	426088	7	NULL	NULL	NULL	NULL	family members	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased penetrance was prominent in family members .
	manualset3
259659	1	426089	7	NULL	NULL	NULL	NULL	Decreased proliferative activity 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased proliferative activity of erythroblasts in granulocytic stem cell leukemia .
	manualset3
259660	2	426089	7	NULL	NULL	NULL	NULL	erythroblasts	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased proliferative activity of erythroblasts in granulocytic stem cell leukemia .
	manualset3
259661	3	426089	7	NULL	NULL	NULL	NULL	granulocytic stem cell leukemia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased proliferative activity of erythroblasts in granulocytic stem cell leukemia .
	manualset3
259662	1	426090	7	NULL	NULL	NULL	NULL	Morphometric characteristics	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Morphometric and immunologic characteristics of lymphocytes of patients with lymphogranulomatosis ) .
	manualset3
259663	2	426090	7	NULL	NULL	NULL	NULL	 immunologic characteristics	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Morphometric and immunologic characteristics of lymphocytes of patients with lymphogranulomatosis ) .
	manualset3
259664	3	426090	7	NULL	NULL	NULL	NULL	lymphocytes	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Morphometric and immunologic characteristics of lymphocytes of patients with lymphogranulomatosis ) .
	manualset3
259665	4	426090	7	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Morphometric and immunologic characteristics of lymphocytes of patients with lymphogranulomatosis ) .
	manualset3
259666	5	426090	7	NULL	NULL	NULL	NULL	lymphogranulomatosis 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Morphometric and immunologic characteristics of lymphocytes of patients with lymphogranulomatosis ) .
	manualset3
259667	1	426091	7	NULL	NULL	NULL	NULL	Decreased responsiveness	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased responsiveness of T-cells to T-cell mitogens , postexercise , may have been the result of decreases in the percentage of T-cells in postexercise mixed lymphocyte cultures rather than depressed cell function .
	manualset3
259668	2	426091	7	NULL	NULL	NULL	NULL	T-cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased responsiveness of T-cells to T-cell mitogens , postexercise , may have been the result of decreases in the percentage of T-cells in postexercise mixed lymphocyte cultures rather than depressed cell function .
	manualset3
259669	3	426091	7	NULL	NULL	NULL	NULL	 T-cell mitogens	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased responsiveness of T-cells to T-cell mitogens , postexercise , may have been the result of decreases in the percentage of T-cells in postexercise mixed lymphocyte cultures rather than depressed cell function .
	manualset3
259670	4	426091	7	NULL	NULL	NULL	NULL	postexercise 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased responsiveness of T-cells to T-cell mitogens , postexercise , may have been the result of decreases in the percentage of T-cells in postexercise mixed lymphocyte cultures rather than depressed cell function .
	manualset3
259671	5	426091	7	NULL	NULL	NULL	NULL	result	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased responsiveness of T-cells to T-cell mitogens , postexercise , may have been the result of decreases in the percentage of T-cells in postexercise mixed lymphocyte cultures rather than depressed cell function .
	manualset3
259672	6	426091	7	NULL	NULL	NULL	NULL	decreases	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased responsiveness of T-cells to T-cell mitogens , postexercise , may have been the result of decreases in the percentage of T-cells in postexercise mixed lymphocyte cultures rather than depressed cell function .
	manualset3
259673	7	426091	7	NULL	NULL	NULL	NULL	 percentage	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased responsiveness of T-cells to T-cell mitogens , postexercise , may have been the result of decreases in the percentage of T-cells in postexercise mixed lymphocyte cultures rather than depressed cell function .
	manualset3
259674	8	426091	7	NULL	NULL	NULL	NULL	 T-cells 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased responsiveness of T-cells to T-cell mitogens , postexercise , may have been the result of decreases in the percentage of T-cells in postexercise mixed lymphocyte cultures rather than depressed cell function .
	manualset3
259675	9	426091	7	NULL	NULL	NULL	NULL	postexercise mixed lymphocyte cultures	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased responsiveness of T-cells to T-cell mitogens , postexercise , may have been the result of decreases in the percentage of T-cells in postexercise mixed lymphocyte cultures rather than depressed cell function .
	manualset3
259676	10	426091	7	NULL	NULL	NULL	NULL	depressed cell function	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased responsiveness of T-cells to T-cell mitogens , postexercise , may have been the result of decreases in the percentage of T-cells in postexercise mixed lymphocyte cultures rather than depressed cell function .
	manualset3
259795	1	426092	7	NULL	NULL	NULL	NULL	Decreased risk	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased risk of stent fracture-related restenosis between paclitaxel-eluting stents and sirolimus eluting stents : results of long-term follow-up .
	manualset3
259796	2	426092	7	NULL	NULL	NULL	NULL	stent fracture-related restenosis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased risk of stent fracture-related restenosis between paclitaxel-eluting stents and sirolimus eluting stents : results of long-term follow-up .
	manualset3
259797	3	426092	7	NULL	NULL	NULL	NULL	paclitaxel-eluting stents	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased risk of stent fracture-related restenosis between paclitaxel-eluting stents and sirolimus eluting stents : results of long-term follow-up .
	manualset3
259798	4	426092	7	NULL	NULL	NULL	NULL	sirolimus eluting stents	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased risk of stent fracture-related restenosis between paclitaxel-eluting stents and sirolimus eluting stents : results of long-term follow-up .
	manualset3
259799	5	426092	7	NULL	NULL	NULL	NULL	 results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased risk of stent fracture-related restenosis between paclitaxel-eluting stents and sirolimus eluting stents : results of long-term follow-up .
	manualset3
259800	6	426092	7	NULL	NULL	NULL	NULL	 long-term follow-up	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased risk of stent fracture-related restenosis between paclitaxel-eluting stents and sirolimus eluting stents : results of long-term follow-up .
	manualset3
259801	1	426093	7	NULL	NULL	NULL	NULL	Decreased spot pecking	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased spot pecking was observed in birds fed on the rations containing 50 g/kg of sugar beet pulp and 200 g/kg of oat hulls .
	manualset3
259802	2	426093	7	NULL	NULL	NULL	NULL	birds	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased spot pecking was observed in birds fed on the rations containing 50 g/kg of sugar beet pulp and 200 g/kg of oat hulls .
	manualset3
259803	3	426093	7	NULL	NULL	NULL	NULL	rations	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased spot pecking was observed in birds fed on the rations containing 50 g/kg of sugar beet pulp and 200 g/kg of oat hulls .
	manualset3
259804	4	426093	7	NULL	NULL	NULL	NULL	50 g/kg	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased spot pecking was observed in birds fed on the rations containing 50 g/kg of sugar beet pulp and 200 g/kg of oat hulls .
	manualset3
259805	5	426093	7	NULL	NULL	NULL	NULL	 sugar beet pulp 	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased spot pecking was observed in birds fed on the rations containing 50 g/kg of sugar beet pulp and 200 g/kg of oat hulls .
	manualset3
259806	6	426093	7	NULL	NULL	NULL	NULL	200 g/kg	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased spot pecking was observed in birds fed on the rations containing 50 g/kg of sugar beet pulp and 200 g/kg of oat hulls .
	manualset3
259807	7	426093	7	NULL	NULL	NULL	NULL	oat hulls	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreased spot pecking was observed in birds fed on the rations containing 50 g/kg of sugar beet pulp and 200 g/kg of oat hulls .
	manualset3
259808	1	426094	7	NULL	NULL	NULL	NULL	bath Cl	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreases in bath Cl caused a significant and reversible increase in cell pH , which was not changed significantly by complete removal of Na from perfusate and bath , but was significantly inhibited by basolateral 4 ' , 5 ' - diisothiocyanostilbene-2 , 2 ' - disulfonic acid .
	manualset3
259809	2	426094	7	NULL	NULL	NULL	NULL	 reversible increase	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreases in bath Cl caused a significant and reversible increase in cell pH , which was not changed significantly by complete removal of Na from perfusate and bath , but was significantly inhibited by basolateral 4 ' , 5 ' - diisothiocyanostilbene-2 , 2 ' - disulfonic acid .
	manualset3
259810	3	426094	7	NULL	NULL	NULL	NULL	cell pH	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreases in bath Cl caused a significant and reversible increase in cell pH , which was not changed significantly by complete removal of Na from perfusate and bath , but was significantly inhibited by basolateral 4 ' , 5 ' - diisothiocyanostilbene-2 , 2 ' - disulfonic acid .
	manualset3
259811	4	426094	7	NULL	NULL	NULL	NULL	complete removal	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreases in bath Cl caused a significant and reversible increase in cell pH , which was not changed significantly by complete removal of Na from perfusate and bath , but was significantly inhibited by basolateral 4 ' , 5 ' - diisothiocyanostilbene-2 , 2 ' - disulfonic acid .
	manualset3
259812	5	426094	7	NULL	NULL	NULL	NULL	Na	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreases in bath Cl caused a significant and reversible increase in cell pH , which was not changed significantly by complete removal of Na from perfusate and bath , but was significantly inhibited by basolateral 4 ' , 5 ' - diisothiocyanostilbene-2 , 2 ' - disulfonic acid .
	manualset3
259813	6	426094	7	NULL	NULL	NULL	NULL	perfusate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreases in bath Cl caused a significant and reversible increase in cell pH , which was not changed significantly by complete removal of Na from perfusate and bath , but was significantly inhibited by basolateral 4 ' , 5 ' - diisothiocyanostilbene-2 , 2 ' - disulfonic acid .
	manualset3
259814	7	426094	7	NULL	NULL	NULL	NULL	bath	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreases in bath Cl caused a significant and reversible increase in cell pH , which was not changed significantly by complete removal of Na from perfusate and bath , but was significantly inhibited by basolateral 4 ' , 5 ' - diisothiocyanostilbene-2 , 2 ' - disulfonic acid .
	manualset3
259815	8	426094	7	NULL	NULL	NULL	NULL	basolateral 4 ' , 5 ' - diisothiocyanostilbene-2 , 2 ' - disulfonic acid	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreases in bath Cl caused a significant and reversible increase in cell pH , which was not changed significantly by complete removal of Na from perfusate and bath , but was significantly inhibited by basolateral 4 ' , 5 ' - diisothiocyanostilbene-2 , 2 ' - disulfonic acid .
	manualset3
259816	1	426095	7	NULL	NULL	NULL	NULL	depressive symptoms	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreases in depressive symptoms were more pronounced for TSF + P than ICBT + P in the 6 months posttreatment .
	manualset3
259817	2	426095	7	NULL	NULL	NULL	NULL	TSF + P than ICBT + P	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreases in depressive symptoms were more pronounced for TSF + P than ICBT + P in the 6 months posttreatment .
	manualset3
259818	3	426095	7	NULL	NULL	NULL	NULL	 6 months	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreases in depressive symptoms were more pronounced for TSF + P than ICBT + P in the 6 months posttreatment .
	manualset3
259819	4	426095	7	NULL	NULL	NULL	NULL	posttreatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreases in depressive symptoms were more pronounced for TSF + P than ICBT + P in the 6 months posttreatment .
	manualset3
259820	1	426096	7	NULL	NULL	NULL	NULL	Decreases	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreases in mean aortic ( 63.6 + / - 3.0 to 54.6 + / - 2.1 mm Hg , p less than 0.05 ) and mean pulmonary artery pressure ( 41.4 + / - 6.2 to 32.0 + / - 6.7 mm Hg , p less than 0.05 ) were also observed .
	manualset3
259821	2	426096	7	NULL	NULL	NULL	NULL	mean aortic pressure	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreases in mean aortic ( 63.6 + / - 3.0 to 54.6 + / - 2.1 mm Hg , p less than 0.05 ) and mean pulmonary artery pressure ( 41.4 + / - 6.2 to 32.0 + / - 6.7 mm Hg , p less than 0.05 ) were also observed .
	manualset3
259822	3	426096	7	NULL	NULL	NULL	NULL	63.6 + / - 3.0 to 54.6 + / - 2.1 mm Hg	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreases in mean aortic ( 63.6 + / - 3.0 to 54.6 + / - 2.1 mm Hg , p less than 0.05 ) and mean pulmonary artery pressure ( 41.4 + / - 6.2 to 32.0 + / - 6.7 mm Hg , p less than 0.05 ) were also observed .
	manualset3
259823	4	426096	7	NULL	NULL	NULL	NULL	p less than 0.05	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreases in mean aortic ( 63.6 + / - 3.0 to 54.6 + / - 2.1 mm Hg , p less than 0.05 ) and mean pulmonary artery pressure ( 41.4 + / - 6.2 to 32.0 + / - 6.7 mm Hg , p less than 0.05 ) were also observed .
	manualset3
259824	5	426096	7	NULL	NULL	NULL	NULL	mean pulmonary artery pressure	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreases in mean aortic ( 63.6 + / - 3.0 to 54.6 + / - 2.1 mm Hg , p less than 0.05 ) and mean pulmonary artery pressure ( 41.4 + / - 6.2 to 32.0 + / - 6.7 mm Hg , p less than 0.05 ) were also observed .
	manualset3
259825	6	426096	7	NULL	NULL	NULL	NULL	41.4 + / - 6.2 to 32.0 + / - 6.7 mm Hg	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreases in mean aortic ( 63.6 + / - 3.0 to 54.6 + / - 2.1 mm Hg , p less than 0.05 ) and mean pulmonary artery pressure ( 41.4 + / - 6.2 to 32.0 + / - 6.7 mm Hg , p less than 0.05 ) were also observed .
	manualset3
259826	7	426096	7	NULL	NULL	NULL	NULL	p less than 0.05 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Decreases in mean aortic ( 63.6 + / - 3.0 to 54.6 + / - 2.1 mm Hg , p less than 0.05 ) and mean pulmonary artery pressure ( 41.4 + / - 6.2 to 32.0 + / - 6.7 mm Hg , p less than 0.05 ) were also observed .
	manualset3
259828	1	426097	7	NULL	NULL	NULL	NULL	Deep brain stimulation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deep brain stimulation for Parkinson 's disease : prevalence of adverse events and need for standardized reporting .
	manualset3
259829	2	426097	7	NULL	NULL	NULL	NULL	Parkinson 's disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deep brain stimulation for Parkinson 's disease : prevalence of adverse events and need for standardized reporting .
	manualset3
259830	3	426097	7	NULL	NULL	NULL	NULL	prevalence 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deep brain stimulation for Parkinson 's disease : prevalence of adverse events and need for standardized reporting .
	manualset3
259831	4	426097	7	NULL	NULL	NULL	NULL	adverse events	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deep brain stimulation for Parkinson 's disease : prevalence of adverse events and need for standardized reporting .
	manualset3
259832	5	426097	7	NULL	NULL	NULL	NULL	standardized reporting	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deep brain stimulation for Parkinson 's disease : prevalence of adverse events and need for standardized reporting .
	manualset3
259835	1	426098	7	NULL	NULL	NULL	NULL	Deep brain stimulation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deep brain stimulation of the subthalamic nucleus : effectiveness in advanced Parkinson 's disease patients previously reliant on apomorphine .
	manualset3
259836	2	426098	7	NULL	NULL	NULL	NULL	subthalamic nucleus	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deep brain stimulation of the subthalamic nucleus : effectiveness in advanced Parkinson 's disease patients previously reliant on apomorphine .
	manualset3
259837	4	426098	7	NULL	NULL	NULL	NULL	advanced Parkinson 's disease patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deep brain stimulation of the subthalamic nucleus : effectiveness in advanced Parkinson 's disease patients previously reliant on apomorphine .
	manualset3
259839	3	426098	7	NULL	NULL	NULL	NULL	effectiveness	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deep brain stimulation of the subthalamic nucleus : effectiveness in advanced Parkinson 's disease patients previously reliant on apomorphine .
	manualset3
259840	5	426098	7	NULL	NULL	NULL	NULL	apomorphine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deep brain stimulation of the subthalamic nucleus : effectiveness in advanced Parkinson 's disease patients previously reliant on apomorphine .
	manualset3
259846	1	426099	7	NULL	NULL	NULL	NULL	Deep tendon reflexes 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deep tendon reflexes demonstrate the homeostasis between the cerebral cortex and the spinal cord .
	manualset3
259848	2	426099	7	NULL	NULL	NULL	NULL	 homeostasis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deep tendon reflexes demonstrate the homeostasis between the cerebral cortex and the spinal cord .
	manualset3
259849	3	426099	7	NULL	NULL	NULL	NULL	cerebral cortex 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deep tendon reflexes demonstrate the homeostasis between the cerebral cortex and the spinal cord .
	manualset3
259850	4	426099	7	NULL	NULL	NULL	NULL	spinal cord	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deep tendon reflexes demonstrate the homeostasis between the cerebral cortex and the spinal cord .
	manualset3
259852	1	426100	7	NULL	NULL	NULL	NULL	Deepened gingival sulci	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deepened gingival sulci , as well as the inconsistency of bleeding after probing associated with labial gingivitis highlighted the problems of using these latter criteria as indicators of health or disease among sheep on the basis of a single examination .
	manualset3
259855	2	426100	7	NULL	NULL	NULL	NULL	 inconsistency	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deepened gingival sulci , as well as the inconsistency of bleeding after probing associated with labial gingivitis highlighted the problems of using these latter criteria as indicators of health or disease among sheep on the basis of a single examination .
	manualset3
259856	3	426100	7	NULL	NULL	NULL	NULL	 bleeding	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deepened gingival sulci , as well as the inconsistency of bleeding after probing associated with labial gingivitis highlighted the problems of using these latter criteria as indicators of health or disease among sheep on the basis of a single examination .
	manualset3
259857	4	426100	7	NULL	NULL	NULL	NULL	labial gingivitis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deepened gingival sulci , as well as the inconsistency of bleeding after probing associated with labial gingivitis highlighted the problems of using these latter criteria as indicators of health or disease among sheep on the basis of a single examination .
	manualset3
259878	5	426100	7	NULL	NULL	NULL	NULL	 problems	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deepened gingival sulci , as well as the inconsistency of bleeding after probing associated with labial gingivitis highlighted the problems of using these latter criteria as indicators of health or disease among sheep on the basis of a single examination .
	manualset3
259879	6	426100	7	NULL	NULL	NULL	NULL	 latter criteria	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deepened gingival sulci , as well as the inconsistency of bleeding after probing associated with labial gingivitis highlighted the problems of using these latter criteria as indicators of health or disease among sheep on the basis of a single examination .
	manualset3
259880	7	426100	7	NULL	NULL	NULL	NULL	indicators 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deepened gingival sulci , as well as the inconsistency of bleeding after probing associated with labial gingivitis highlighted the problems of using these latter criteria as indicators of health or disease among sheep on the basis of a single examination .
	manualset3
259881	8	426100	7	NULL	NULL	NULL	NULL	health	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deepened gingival sulci , as well as the inconsistency of bleeding after probing associated with labial gingivitis highlighted the problems of using these latter criteria as indicators of health or disease among sheep on the basis of a single examination .
	manualset3
259882	9	426100	7	NULL	NULL	NULL	NULL	disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deepened gingival sulci , as well as the inconsistency of bleeding after probing associated with labial gingivitis highlighted the problems of using these latter criteria as indicators of health or disease among sheep on the basis of a single examination .
	manualset3
259883	10	426100	7	NULL	NULL	NULL	NULL	sheep	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deepened gingival sulci , as well as the inconsistency of bleeding after probing associated with labial gingivitis highlighted the problems of using these latter criteria as indicators of health or disease among sheep on the basis of a single examination .
	manualset3
259884	11	426100	7	NULL	NULL	NULL	NULL	 basis	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deepened gingival sulci , as well as the inconsistency of bleeding after probing associated with labial gingivitis highlighted the problems of using these latter criteria as indicators of health or disease among sheep on the basis of a single examination .
	manualset3
259885	12	426100	7	NULL	NULL	NULL	NULL	single examination	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deepened gingival sulci , as well as the inconsistency of bleeding after probing associated with labial gingivitis highlighted the problems of using these latter criteria as indicators of health or disease among sheep on the basis of a single examination .
	manualset3
259886	1	426101	7	NULL	NULL	NULL	NULL	Defects	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects in X-linked phosphoribosylpyrophosphate synthetase 1 ( PRPS1 ) manifest as follows : ( 1 ) PRS-I enzyme `` superactivity '' ( gain-of-function mutations affecting allosteric regions ) ; ( 2 ) PRS-I overexpression ( which may be linked to miRNA mutation ) ; ( 3 ) severe PRS-I deficiency/Arts syndrome ( missense mutations producing loss-of-function ) ; ( 4 ) moderate PRS-I deficiency/Charcot-Marie-Tooth disease-5 ( less severe loss-of-function mutations ) ; and ( 5 ) mild PRS-I deficiency/Deafness -2 ( mutations producing slight destabilization ) .
	manualset3
259887	2	426101	7	NULL	NULL	NULL	NULL	X-linked phosphoribosylpyrophosphate synthetase 1 ( PRPS1 )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects in X-linked phosphoribosylpyrophosphate synthetase 1 ( PRPS1 ) manifest as follows : ( 1 ) PRS-I enzyme `` superactivity '' ( gain-of-function mutations affecting allosteric regions ) ; ( 2 ) PRS-I overexpression ( which may be linked to miRNA mutation ) ; ( 3 ) severe PRS-I deficiency/Arts syndrome ( missense mutations producing loss-of-function ) ; ( 4 ) moderate PRS-I deficiency/Charcot-Marie-Tooth disease-5 ( less severe loss-of-function mutations ) ; and ( 5 ) mild PRS-I deficiency/Deafness -2 ( mutations producing slight destabilization ) .
	manualset3
259888	3	426101	7	NULL	NULL	NULL	NULL	PRS-I enzyme `` superactivity '' 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects in X-linked phosphoribosylpyrophosphate synthetase 1 ( PRPS1 ) manifest as follows : ( 1 ) PRS-I enzyme `` superactivity '' ( gain-of-function mutations affecting allosteric regions ) ; ( 2 ) PRS-I overexpression ( which may be linked to miRNA mutation ) ; ( 3 ) severe PRS-I deficiency/Arts syndrome ( missense mutations producing loss-of-function ) ; ( 4 ) moderate PRS-I deficiency/Charcot-Marie-Tooth disease-5 ( less severe loss-of-function mutations ) ; and ( 5 ) mild PRS-I deficiency/Deafness -2 ( mutations producing slight destabilization ) .
	manualset3
259889	4	426101	7	NULL	NULL	NULL	NULL	gain-of-function mutations	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects in X-linked phosphoribosylpyrophosphate synthetase 1 ( PRPS1 ) manifest as follows : ( 1 ) PRS-I enzyme `` superactivity '' ( gain-of-function mutations affecting allosteric regions ) ; ( 2 ) PRS-I overexpression ( which may be linked to miRNA mutation ) ; ( 3 ) severe PRS-I deficiency/Arts syndrome ( missense mutations producing loss-of-function ) ; ( 4 ) moderate PRS-I deficiency/Charcot-Marie-Tooth disease-5 ( less severe loss-of-function mutations ) ; and ( 5 ) mild PRS-I deficiency/Deafness -2 ( mutations producing slight destabilization ) .
	manualset3
259890	5	426101	7	NULL	NULL	NULL	NULL	allosteric regions	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects in X-linked phosphoribosylpyrophosphate synthetase 1 ( PRPS1 ) manifest as follows : ( 1 ) PRS-I enzyme `` superactivity '' ( gain-of-function mutations affecting allosteric regions ) ; ( 2 ) PRS-I overexpression ( which may be linked to miRNA mutation ) ; ( 3 ) severe PRS-I deficiency/Arts syndrome ( missense mutations producing loss-of-function ) ; ( 4 ) moderate PRS-I deficiency/Charcot-Marie-Tooth disease-5 ( less severe loss-of-function mutations ) ; and ( 5 ) mild PRS-I deficiency/Deafness -2 ( mutations producing slight destabilization ) .
	manualset3
259891	6	426101	7	NULL	NULL	NULL	NULL	PRS-I overexpression 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects in X-linked phosphoribosylpyrophosphate synthetase 1 ( PRPS1 ) manifest as follows : ( 1 ) PRS-I enzyme `` superactivity '' ( gain-of-function mutations affecting allosteric regions ) ; ( 2 ) PRS-I overexpression ( which may be linked to miRNA mutation ) ; ( 3 ) severe PRS-I deficiency/Arts syndrome ( missense mutations producing loss-of-function ) ; ( 4 ) moderate PRS-I deficiency/Charcot-Marie-Tooth disease-5 ( less severe loss-of-function mutations ) ; and ( 5 ) mild PRS-I deficiency/Deafness -2 ( mutations producing slight destabilization ) .
	manualset3
259892	7	426101	7	NULL	NULL	NULL	NULL	 miRNA mutation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects in X-linked phosphoribosylpyrophosphate synthetase 1 ( PRPS1 ) manifest as follows : ( 1 ) PRS-I enzyme `` superactivity '' ( gain-of-function mutations affecting allosteric regions ) ; ( 2 ) PRS-I overexpression ( which may be linked to miRNA mutation ) ; ( 3 ) severe PRS-I deficiency/Arts syndrome ( missense mutations producing loss-of-function ) ; ( 4 ) moderate PRS-I deficiency/Charcot-Marie-Tooth disease-5 ( less severe loss-of-function mutations ) ; and ( 5 ) mild PRS-I deficiency/Deafness -2 ( mutations producing slight destabilization ) .
	manualset3
259893	8	426101	7	NULL	NULL	NULL	NULL	severe PRS-I deficiency	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects in X-linked phosphoribosylpyrophosphate synthetase 1 ( PRPS1 ) manifest as follows : ( 1 ) PRS-I enzyme `` superactivity '' ( gain-of-function mutations affecting allosteric regions ) ; ( 2 ) PRS-I overexpression ( which may be linked to miRNA mutation ) ; ( 3 ) severe PRS-I deficiency/Arts syndrome ( missense mutations producing loss-of-function ) ; ( 4 ) moderate PRS-I deficiency/Charcot-Marie-Tooth disease-5 ( less severe loss-of-function mutations ) ; and ( 5 ) mild PRS-I deficiency/Deafness -2 ( mutations producing slight destabilization ) .
	manualset3
259894	9	426101	7	NULL	NULL	NULL	NULL	Arts syndrome 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects in X-linked phosphoribosylpyrophosphate synthetase 1 ( PRPS1 ) manifest as follows : ( 1 ) PRS-I enzyme `` superactivity '' ( gain-of-function mutations affecting allosteric regions ) ; ( 2 ) PRS-I overexpression ( which may be linked to miRNA mutation ) ; ( 3 ) severe PRS-I deficiency/Arts syndrome ( missense mutations producing loss-of-function ) ; ( 4 ) moderate PRS-I deficiency/Charcot-Marie-Tooth disease-5 ( less severe loss-of-function mutations ) ; and ( 5 ) mild PRS-I deficiency/Deafness -2 ( mutations producing slight destabilization ) .
	manualset3
259895	10	426101	7	NULL	NULL	NULL	NULL	 missense mutations	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects in X-linked phosphoribosylpyrophosphate synthetase 1 ( PRPS1 ) manifest as follows : ( 1 ) PRS-I enzyme `` superactivity '' ( gain-of-function mutations affecting allosteric regions ) ; ( 2 ) PRS-I overexpression ( which may be linked to miRNA mutation ) ; ( 3 ) severe PRS-I deficiency/Arts syndrome ( missense mutations producing loss-of-function ) ; ( 4 ) moderate PRS-I deficiency/Charcot-Marie-Tooth disease-5 ( less severe loss-of-function mutations ) ; and ( 5 ) mild PRS-I deficiency/Deafness -2 ( mutations producing slight destabilization ) .
	manualset3
259896	11	426101	7	NULL	NULL	NULL	NULL	loss-of-function 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects in X-linked phosphoribosylpyrophosphate synthetase 1 ( PRPS1 ) manifest as follows : ( 1 ) PRS-I enzyme `` superactivity '' ( gain-of-function mutations affecting allosteric regions ) ; ( 2 ) PRS-I overexpression ( which may be linked to miRNA mutation ) ; ( 3 ) severe PRS-I deficiency/Arts syndrome ( missense mutations producing loss-of-function ) ; ( 4 ) moderate PRS-I deficiency/Charcot-Marie-Tooth disease-5 ( less severe loss-of-function mutations ) ; and ( 5 ) mild PRS-I deficiency/Deafness -2 ( mutations producing slight destabilization ) .
	manualset3
259897	12	426101	7	NULL	NULL	NULL	NULL	moderate PRS-I deficiency	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects in X-linked phosphoribosylpyrophosphate synthetase 1 ( PRPS1 ) manifest as follows : ( 1 ) PRS-I enzyme `` superactivity '' ( gain-of-function mutations affecting allosteric regions ) ; ( 2 ) PRS-I overexpression ( which may be linked to miRNA mutation ) ; ( 3 ) severe PRS-I deficiency/Arts syndrome ( missense mutations producing loss-of-function ) ; ( 4 ) moderate PRS-I deficiency/Charcot-Marie-Tooth disease-5 ( less severe loss-of-function mutations ) ; and ( 5 ) mild PRS-I deficiency/Deafness -2 ( mutations producing slight destabilization ) .
	manualset3
259898	13	426101	7	NULL	NULL	NULL	NULL	Charcot-Marie-Tooth disease-5 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects in X-linked phosphoribosylpyrophosphate synthetase 1 ( PRPS1 ) manifest as follows : ( 1 ) PRS-I enzyme `` superactivity '' ( gain-of-function mutations affecting allosteric regions ) ; ( 2 ) PRS-I overexpression ( which may be linked to miRNA mutation ) ; ( 3 ) severe PRS-I deficiency/Arts syndrome ( missense mutations producing loss-of-function ) ; ( 4 ) moderate PRS-I deficiency/Charcot-Marie-Tooth disease-5 ( less severe loss-of-function mutations ) ; and ( 5 ) mild PRS-I deficiency/Deafness -2 ( mutations producing slight destabilization ) .
	manualset3
259899	14	426101	7	NULL	NULL	NULL	NULL	 loss-of-function mutations 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects in X-linked phosphoribosylpyrophosphate synthetase 1 ( PRPS1 ) manifest as follows : ( 1 ) PRS-I enzyme `` superactivity '' ( gain-of-function mutations affecting allosteric regions ) ; ( 2 ) PRS-I overexpression ( which may be linked to miRNA mutation ) ; ( 3 ) severe PRS-I deficiency/Arts syndrome ( missense mutations producing loss-of-function ) ; ( 4 ) moderate PRS-I deficiency/Charcot-Marie-Tooth disease-5 ( less severe loss-of-function mutations ) ; and ( 5 ) mild PRS-I deficiency/Deafness -2 ( mutations producing slight destabilization ) .
	manualset3
259900	15	426101	7	NULL	NULL	NULL	NULL	mild PRS-I deficiency	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects in X-linked phosphoribosylpyrophosphate synthetase 1 ( PRPS1 ) manifest as follows : ( 1 ) PRS-I enzyme `` superactivity '' ( gain-of-function mutations affecting allosteric regions ) ; ( 2 ) PRS-I overexpression ( which may be linked to miRNA mutation ) ; ( 3 ) severe PRS-I deficiency/Arts syndrome ( missense mutations producing loss-of-function ) ; ( 4 ) moderate PRS-I deficiency/Charcot-Marie-Tooth disease-5 ( less severe loss-of-function mutations ) ; and ( 5 ) mild PRS-I deficiency/Deafness -2 ( mutations producing slight destabilization ) .
	manualset3
259901	16	426101	7	NULL	NULL	NULL	NULL	Deafness -2	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects in X-linked phosphoribosylpyrophosphate synthetase 1 ( PRPS1 ) manifest as follows : ( 1 ) PRS-I enzyme `` superactivity '' ( gain-of-function mutations affecting allosteric regions ) ; ( 2 ) PRS-I overexpression ( which may be linked to miRNA mutation ) ; ( 3 ) severe PRS-I deficiency/Arts syndrome ( missense mutations producing loss-of-function ) ; ( 4 ) moderate PRS-I deficiency/Charcot-Marie-Tooth disease-5 ( less severe loss-of-function mutations ) ; and ( 5 ) mild PRS-I deficiency/Deafness -2 ( mutations producing slight destabilization ) .
	manualset3
259902	17	426101	7	NULL	NULL	NULL	NULL	mutations	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects in X-linked phosphoribosylpyrophosphate synthetase 1 ( PRPS1 ) manifest as follows : ( 1 ) PRS-I enzyme `` superactivity '' ( gain-of-function mutations affecting allosteric regions ) ; ( 2 ) PRS-I overexpression ( which may be linked to miRNA mutation ) ; ( 3 ) severe PRS-I deficiency/Arts syndrome ( missense mutations producing loss-of-function ) ; ( 4 ) moderate PRS-I deficiency/Charcot-Marie-Tooth disease-5 ( less severe loss-of-function mutations ) ; and ( 5 ) mild PRS-I deficiency/Deafness -2 ( mutations producing slight destabilization ) .
	manualset3
259903	18	426101	7	NULL	NULL	NULL	NULL	slight destabilization 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects in X-linked phosphoribosylpyrophosphate synthetase 1 ( PRPS1 ) manifest as follows : ( 1 ) PRS-I enzyme `` superactivity '' ( gain-of-function mutations affecting allosteric regions ) ; ( 2 ) PRS-I overexpression ( which may be linked to miRNA mutation ) ; ( 3 ) severe PRS-I deficiency/Arts syndrome ( missense mutations producing loss-of-function ) ; ( 4 ) moderate PRS-I deficiency/Charcot-Marie-Tooth disease-5 ( less severe loss-of-function mutations ) ; and ( 5 ) mild PRS-I deficiency/Deafness -2 ( mutations producing slight destabilization ) .
	manualset3
259904	1	426102	7	NULL	NULL	NULL	NULL	Defects	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects in spermatogenesis have been found associated with deletions of different portions of Y chromosome long arm ( Yq ) , suggesting the presence of the azoospermia factor in the control of spermatogenesis .
	manualset3
259905	2	426102	7	NULL	NULL	NULL	NULL	spermatogenesis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects in spermatogenesis have been found associated with deletions of different portions of Y chromosome long arm ( Yq ) , suggesting the presence of the azoospermia factor in the control of spermatogenesis .
	manualset3
259906	3	426102	7	NULL	NULL	NULL	NULL	deletions	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects in spermatogenesis have been found associated with deletions of different portions of Y chromosome long arm ( Yq ) , suggesting the presence of the azoospermia factor in the control of spermatogenesis .
	manualset3
259907	4	426102	7	NULL	NULL	NULL	NULL	different portions	Chromosome												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects in spermatogenesis have been found associated with deletions of different portions of Y chromosome long arm ( Yq ) , suggesting the presence of the azoospermia factor in the control of spermatogenesis .
	manualset3
259908	5	426102	7	NULL	NULL	NULL	NULL	Y chromosome long arm ( Yq ) 	Chromosome												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects in spermatogenesis have been found associated with deletions of different portions of Y chromosome long arm ( Yq ) , suggesting the presence of the azoospermia factor in the control of spermatogenesis .
	manualset3
259909	6	426102	7	NULL	NULL	NULL	NULL	presence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects in spermatogenesis have been found associated with deletions of different portions of Y chromosome long arm ( Yq ) , suggesting the presence of the azoospermia factor in the control of spermatogenesis .
	manualset3
259910	7	426102	7	NULL	NULL	NULL	NULL	azoospermia factor 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects in spermatogenesis have been found associated with deletions of different portions of Y chromosome long arm ( Yq ) , suggesting the presence of the azoospermia factor in the control of spermatogenesis .
	manualset3
259911	8	426102	7	NULL	NULL	NULL	NULL	control 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects in spermatogenesis have been found associated with deletions of different portions of Y chromosome long arm ( Yq ) , suggesting the presence of the azoospermia factor in the control of spermatogenesis .
	manualset3
259912	9	426102	7	NULL	NULL	NULL	NULL	spermatogenesis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects in spermatogenesis have been found associated with deletions of different portions of Y chromosome long arm ( Yq ) , suggesting the presence of the azoospermia factor in the control of spermatogenesis .
	manualset3
259913	1	426103	7	NULL	NULL	NULL	NULL	Defects	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects of mitochondrial DNA ( mtDNA ) maintenance have recently been associated with inherited neurodegenerative and muscle diseases and the aging process .
	manualset3
259914	2	426103	7	NULL	NULL	NULL	NULL	mitochondrial DNA ( mtDNA ) maintenance	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects of mitochondrial DNA ( mtDNA ) maintenance have recently been associated with inherited neurodegenerative and muscle diseases and the aging process .
	manualset3
259915	3	426103	7	NULL	NULL	NULL	NULL	inherited neurodegenerative diseases	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects of mitochondrial DNA ( mtDNA ) maintenance have recently been associated with inherited neurodegenerative and muscle diseases and the aging process .
	manualset3
259916	4	426103	7	NULL	NULL	NULL	NULL	muscle diseases	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects of mitochondrial DNA ( mtDNA ) maintenance have recently been associated with inherited neurodegenerative and muscle diseases and the aging process .
	manualset3
259917	5	426103	7	NULL	NULL	NULL	NULL	aging process	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects of mitochondrial DNA ( mtDNA ) maintenance have recently been associated with inherited neurodegenerative and muscle diseases and the aging process .
	manualset3
259918	1	426104	7	NULL	NULL	NULL	NULL	Defects	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects of renal tubular function in the nephrotic syndrome ; observations on a nephrotic child with aminoaciduria , glycosuria , polyuria , tubular acidosis , and potassium depletion .
	manualset3
259919	2	426104	7	NULL	NULL	NULL	NULL	renal tubular function	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects of renal tubular function in the nephrotic syndrome ; observations on a nephrotic child with aminoaciduria , glycosuria , polyuria , tubular acidosis , and potassium depletion .
	manualset3
259920	3	426104	7	NULL	NULL	NULL	NULL	nephrotic syndrome	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects of renal tubular function in the nephrotic syndrome ; observations on a nephrotic child with aminoaciduria , glycosuria , polyuria , tubular acidosis , and potassium depletion .
	manualset3
259921	4	426104	7	NULL	NULL	NULL	NULL	observations 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects of renal tubular function in the nephrotic syndrome ; observations on a nephrotic child with aminoaciduria , glycosuria , polyuria , tubular acidosis , and potassium depletion .
	manualset3
259922	5	426104	7	NULL	NULL	NULL	NULL	 nephrotic child	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects of renal tubular function in the nephrotic syndrome ; observations on a nephrotic child with aminoaciduria , glycosuria , polyuria , tubular acidosis , and potassium depletion .
	manualset3
259923	6	426104	7	NULL	NULL	NULL	NULL	aminoaciduria 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects of renal tubular function in the nephrotic syndrome ; observations on a nephrotic child with aminoaciduria , glycosuria , polyuria , tubular acidosis , and potassium depletion .
	manualset3
259924	7	426104	7	NULL	NULL	NULL	NULL	glycosuria	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects of renal tubular function in the nephrotic syndrome ; observations on a nephrotic child with aminoaciduria , glycosuria , polyuria , tubular acidosis , and potassium depletion .
	manualset3
259925	8	426104	7	NULL	NULL	NULL	NULL	 polyuria	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects of renal tubular function in the nephrotic syndrome ; observations on a nephrotic child with aminoaciduria , glycosuria , polyuria , tubular acidosis , and potassium depletion .
	manualset3
259926	9	426104	7	NULL	NULL	NULL	NULL	tubular acidosis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects of renal tubular function in the nephrotic syndrome ; observations on a nephrotic child with aminoaciduria , glycosuria , polyuria , tubular acidosis , and potassium depletion .
	manualset3
259927	10	426104	7	NULL	NULL	NULL	NULL	potassium depletion	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defects of renal tubular function in the nephrotic syndrome ; observations on a nephrotic child with aminoaciduria , glycosuria , polyuria , tubular acidosis , and potassium depletion .
	manualset3
259928	1	426105	7	NULL	NULL	NULL	NULL	Deferoxamine-induced attenuation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deferoxamine-induced attenuation of brain edema and neurological deficits in a rat model of intracerebral hemorrhage .
	manualset3
259929	2	426105	7	NULL	NULL	NULL	NULL	brain edema	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deferoxamine-induced attenuation of brain edema and neurological deficits in a rat model of intracerebral hemorrhage .
	manualset3
259930	3	426105	7	NULL	NULL	NULL	NULL	neurological deficits	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deferoxamine-induced attenuation of brain edema and neurological deficits in a rat model of intracerebral hemorrhage .
	manualset3
259931	4	426105	7	NULL	NULL	NULL	NULL	 rat model 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deferoxamine-induced attenuation of brain edema and neurological deficits in a rat model of intracerebral hemorrhage .
	manualset3
259932	5	426105	7	NULL	NULL	NULL	NULL	intracerebral hemorrhage	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deferoxamine-induced attenuation of brain edema and neurological deficits in a rat model of intracerebral hemorrhage .
	manualset3
259933	1	426106	7	NULL	NULL	NULL	NULL	Deficiency 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deficiency in 15-hydroxyprostaglandin dehydrogenase activity after unilateral ureteral obstruction of the dog kidney .
	manualset3
259934	2	426106	7	NULL	NULL	NULL	NULL	15-hydroxyprostaglandin dehydrogenase activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deficiency in 15-hydroxyprostaglandin dehydrogenase activity after unilateral ureteral obstruction of the dog kidney .
	manualset3
259935	3	426106	7	NULL	NULL	NULL	NULL	unilateral ureteral obstruction	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deficiency in 15-hydroxyprostaglandin dehydrogenase activity after unilateral ureteral obstruction of the dog kidney .
	manualset3
259936	4	426106	7	NULL	NULL	NULL	NULL	dog kidney	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deficiency in 15-hydroxyprostaglandin dehydrogenase activity after unilateral ureteral obstruction of the dog kidney .
	manualset3
259937	1	426107	7	NULL	NULL	NULL	NULL	Deficits	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deficits , however , are observed in their lower internal consistency and relative uncertainty and in higher response polarization and perseveration .
	manualset3
259938	2	426107	7	NULL	NULL	NULL	NULL	lower internal consistency	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deficits , however , are observed in their lower internal consistency and relative uncertainty and in higher response polarization and perseveration .
	manualset3
259939	3	426107	7	NULL	NULL	NULL	NULL	relative uncertainty 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deficits , however , are observed in their lower internal consistency and relative uncertainty and in higher response polarization and perseveration .
	manualset3
259940	4	426107	7	NULL	NULL	NULL	NULL	higher response polarization	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deficits , however , are observed in their lower internal consistency and relative uncertainty and in higher response polarization and perseveration .
	manualset3
259941	5	426107	7	NULL	NULL	NULL	NULL	perseveration	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deficits , however , are observed in their lower internal consistency and relative uncertainty and in higher response polarization and perseveration .
	manualset3
259942	1	426108	7	NULL	NULL	NULL	NULL	Deficits	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deficits in prospective memory following damage to the prefrontal cortex .
	manualset3
259943	2	426108	7	NULL	NULL	NULL	NULL	prospective memory	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deficits in prospective memory following damage to the prefrontal cortex .
	manualset3
259944	3	426108	7	NULL	NULL	NULL	NULL	damage	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deficits in prospective memory following damage to the prefrontal cortex .
	manualset3
259945	4	426108	7	NULL	NULL	NULL	NULL	prefrontal cortex	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deficits in prospective memory following damage to the prefrontal cortex .
	manualset3
259946	1	426109	7	NULL	NULL	NULL	NULL	Multiple dental cysts	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Multiple dental cysts or polycystic adamantinoma ) .
	manualset3
259947	2	426109	7	NULL	NULL	NULL	NULL	polycystic adamantinoma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Multiple dental cysts or polycystic adamantinoma ) .
	manualset3
259948	1	426110	7	NULL	NULL	NULL	NULL	fluctuation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defining both fluctuation in breast-milk virus level over time and how breast-milk virus correlates with mother-to-child transmission is important for establishing effective interventions .
	manualset3
259949	2	426110	7	NULL	NULL	NULL	NULL	breast-milk virus level	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defining both fluctuation in breast-milk virus level over time and how breast-milk virus correlates with mother-to-child transmission is important for establishing effective interventions .
	manualset3
259950	3	426110	7	NULL	NULL	NULL	NULL	 time	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defining both fluctuation in breast-milk virus level over time and how breast-milk virus correlates with mother-to-child transmission is important for establishing effective interventions .
	manualset3
259951	4	426110	7	NULL	NULL	NULL	NULL	breast-milk virus	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defining both fluctuation in breast-milk virus level over time and how breast-milk virus correlates with mother-to-child transmission is important for establishing effective interventions .
	manualset3
259952	5	426110	7	NULL	NULL	NULL	NULL	 mother-to-child transmission	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defining both fluctuation in breast-milk virus level over time and how breast-milk virus correlates with mother-to-child transmission is important for establishing effective interventions .
	manualset3
259953	6	426110	7	NULL	NULL	NULL	NULL	effective interventions	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Defining both fluctuation in breast-milk virus level over time and how breast-milk virus correlates with mother-to-child transmission is important for establishing effective interventions .
	manualset3
259954	1	426111	7	NULL	NULL	NULL	NULL	Definition 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Definition , review , orientation studies on consistency and structural stability ) .
	manualset3
259955	2	426111	7	NULL	NULL	NULL	NULL	review	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Definition , review , orientation studies on consistency and structural stability ) .
	manualset3
259956	3	426111	7	NULL	NULL	NULL	NULL	orientation studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Definition , review , orientation studies on consistency and structural stability ) .
	manualset3
259957	4	426111	7	NULL	NULL	NULL	NULL	consistency	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Definition , review , orientation studies on consistency and structural stability ) .
	manualset3
259958	5	426111	7	NULL	NULL	NULL	NULL	structural stability	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Definition , review , orientation studies on consistency and structural stability ) .
	manualset3
259959	1	426112	7	NULL	NULL	NULL	NULL	Definition	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Definition of therapy-resistant schizophrenia and its assessment .
	manualset3
259960	2	426112	7	NULL	NULL	NULL	NULL	therapy-resistant schizophrenia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Definition of therapy-resistant schizophrenia and its assessment .
	manualset3
259961	3	426112	7	NULL	NULL	NULL	NULL	assessment	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Definition of therapy-resistant schizophrenia and its assessment .
	manualset3
259962	1	426113	7	NULL	NULL	NULL	NULL	organ-sparing treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Definitive organ-sparing treatment of anal canal cancer : can we afford to question it ?
	manualset3
259963	2	426113	7	NULL	NULL	NULL	NULL	anal canal cancer	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Definitive organ-sparing treatment of anal canal cancer : can we afford to question it ?
	manualset3
259964	1	426114	7	NULL	NULL	NULL	NULL	Deformation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deformation of SUVs is revealed by comparing the quenching of the donors to calculations of FRET between a perfectly spherical shell and a flat surface containing complementary fluorophores .
	manualset3
259965	2	426114	7	NULL	NULL	NULL	NULL	SUVs	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deformation of SUVs is revealed by comparing the quenching of the donors to calculations of FRET between a perfectly spherical shell and a flat surface containing complementary fluorophores .
	manualset3
259966	3	426114	7	NULL	NULL	NULL	NULL	quenching	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deformation of SUVs is revealed by comparing the quenching of the donors to calculations of FRET between a perfectly spherical shell and a flat surface containing complementary fluorophores .
	manualset3
259967	4	426114	7	NULL	NULL	NULL	NULL	donors	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deformation of SUVs is revealed by comparing the quenching of the donors to calculations of FRET between a perfectly spherical shell and a flat surface containing complementary fluorophores .
	manualset3
259968	5	426114	7	NULL	NULL	NULL	NULL	 calculations 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deformation of SUVs is revealed by comparing the quenching of the donors to calculations of FRET between a perfectly spherical shell and a flat surface containing complementary fluorophores .
	manualset3
259969	6	426114	7	NULL	NULL	NULL	NULL	FRET	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deformation of SUVs is revealed by comparing the quenching of the donors to calculations of FRET between a perfectly spherical shell and a flat surface containing complementary fluorophores .
	manualset3
259970	7	426114	7	NULL	NULL	NULL	NULL	perfectly spherical shell	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deformation of SUVs is revealed by comparing the quenching of the donors to calculations of FRET between a perfectly spherical shell and a flat surface containing complementary fluorophores .
	manualset3
259971	8	426114	7	NULL	NULL	NULL	NULL	flat surface	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deformation of SUVs is revealed by comparing the quenching of the donors to calculations of FRET between a perfectly spherical shell and a flat surface containing complementary fluorophores .
	manualset3
259972	9	426114	7	NULL	NULL	NULL	NULL	complementary fluorophores	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deformation of SUVs is revealed by comparing the quenching of the donors to calculations of FRET between a perfectly spherical shell and a flat surface containing complementary fluorophores .
	manualset3
259973	1	426115	7	NULL	NULL	NULL	NULL	Degenerating germ cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Degenerating germ cells identified by histology were present at certain stages of spermatogenesis after 2 weeks of antagonist treatment .
	manualset3
259974	2	426115	7	NULL	NULL	NULL	NULL	histology	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Degenerating germ cells identified by histology were present at certain stages of spermatogenesis after 2 weeks of antagonist treatment .
	manualset3
259975	3	426115	7	NULL	NULL	NULL	NULL	certain stages	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Degenerating germ cells identified by histology were present at certain stages of spermatogenesis after 2 weeks of antagonist treatment .
	manualset3
259976	4	426115	7	NULL	NULL	NULL	NULL	spermatogenesis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Degenerating germ cells identified by histology were present at certain stages of spermatogenesis after 2 weeks of antagonist treatment .
	manualset3
259977	5	426115	7	NULL	NULL	NULL	NULL	2 weeks	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Degenerating germ cells identified by histology were present at certain stages of spermatogenesis after 2 weeks of antagonist treatment .
	manualset3
259978	6	426115	7	NULL	NULL	NULL	NULL	antagonist treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Degenerating germ cells identified by histology were present at certain stages of spermatogenesis after 2 weeks of antagonist treatment .
	manualset3
259979	1	426116	7	NULL	NULL	NULL	NULL	 Mumps vaccination	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Mumps vaccination and morbidity in the Finnish Army 1967-70 ) .
	manualset3
259980	2	426116	7	NULL	NULL	NULL	NULL	morbidity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Mumps vaccination and morbidity in the Finnish Army 1967-70 ) .
	manualset3
259981	3	426116	7	NULL	NULL	NULL	NULL	 Finnish Army	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Mumps vaccination and morbidity in the Finnish Army 1967-70 ) .
	manualset3
259982	4	426116	7	NULL	NULL	NULL	NULL	1967-70	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Mumps vaccination and morbidity in the Finnish Army 1967-70 ) .
	manualset3
259983	1	426117	7	NULL	NULL	NULL	NULL	Degeneration	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Degeneration in central and peripheral nervous systems produced by pure n-hexane : an experimental study .
	manualset3
259984	2	426117	7	NULL	NULL	NULL	NULL	central nervous system	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Degeneration in central and peripheral nervous systems produced by pure n-hexane : an experimental study .
	manualset3
259985	3	426117	7	NULL	NULL	NULL	NULL	peripheral nervous systems	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Degeneration in central and peripheral nervous systems produced by pure n-hexane : an experimental study .
	manualset3
259986	4	426117	7	NULL	NULL	NULL	NULL	 pure n-hexane	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Degeneration in central and peripheral nervous systems produced by pure n-hexane : an experimental study .
	manualset3
259987	5	426117	7	NULL	NULL	NULL	NULL	experimental study 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Degeneration in central and peripheral nervous systems produced by pure n-hexane : an experimental study .
	manualset3
259988	1	426118	7	NULL	NULL	NULL	NULL	Degradation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Degradation of rutin by Aspergillus flavus .
	manualset3
259989	2	426118	7	NULL	NULL	NULL	NULL	rutin 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Degradation of rutin by Aspergillus flavus .
	manualset3
259990	3	426118	7	NULL	NULL	NULL	NULL	Aspergillus flavus	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Degradation of rutin by Aspergillus flavus .
	manualset3
259991	1	426119	7	NULL	NULL	NULL	NULL	Degradation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Degradation of the cartilage proteoglycan aggrecan is one of the earliest events that occurs in association with osteoarthritis .
	manualset3
259992	2	426119	7	NULL	NULL	NULL	NULL	cartilage proteoglycan aggrecan	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Degradation of the cartilage proteoglycan aggrecan is one of the earliest events that occurs in association with osteoarthritis .
	manualset3
259993	3	426119	7	NULL	NULL	NULL	NULL	one	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Degradation of the cartilage proteoglycan aggrecan is one of the earliest events that occurs in association with osteoarthritis .
	manualset3
259994	4	426119	7	NULL	NULL	NULL	NULL	earliest events	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Degradation of the cartilage proteoglycan aggrecan is one of the earliest events that occurs in association with osteoarthritis .
	manualset3
259995	5	426119	7	NULL	NULL	NULL	NULL	association	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Degradation of the cartilage proteoglycan aggrecan is one of the earliest events that occurs in association with osteoarthritis .
	manualset3
259996	6	426119	7	NULL	NULL	NULL	NULL	osteoarthritis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Degradation of the cartilage proteoglycan aggrecan is one of the earliest events that occurs in association with osteoarthritis .
	manualset3
259997	1	426120	7	NULL	NULL	NULL	NULL	Deh4p	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deh4p has apparent K ( m ) s of 5.5 and 8.9 muM and V ( max ) s of 9.1 and 23.1 nmol mg ( -1 ) min ( -1 ) for acetate and MCA , respectively .
	manualset3
259998	2	426120	7	NULL	NULL	NULL	NULL	K ( m ) s	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deh4p has apparent K ( m ) s of 5.5 and 8.9 muM and V ( max ) s of 9.1 and 23.1 nmol mg ( -1 ) min ( -1 ) for acetate and MCA , respectively .
	manualset3
259999	3	426120	7	NULL	NULL	NULL	NULL	 5.5 muM	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deh4p has apparent K ( m ) s of 5.5 and 8.9 muM and V ( max ) s of 9.1 and 23.1 nmol mg ( -1 ) min ( -1 ) for acetate and MCA , respectively .
	manualset3
260000	4	426120	7	NULL	NULL	NULL	NULL	8.9 muM	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deh4p has apparent K ( m ) s of 5.5 and 8.9 muM and V ( max ) s of 9.1 and 23.1 nmol mg ( -1 ) min ( -1 ) for acetate and MCA , respectively .
	manualset3
260001	5	426120	7	NULL	NULL	NULL	NULL	V ( max ) s	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deh4p has apparent K ( m ) s of 5.5 and 8.9 muM and V ( max ) s of 9.1 and 23.1 nmol mg ( -1 ) min ( -1 ) for acetate and MCA , respectively .
	manualset3
260002	6	426120	7	NULL	NULL	NULL	NULL	9.1 nmol mg ( -1 ) min ( -1 )	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deh4p has apparent K ( m ) s of 5.5 and 8.9 muM and V ( max ) s of 9.1 and 23.1 nmol mg ( -1 ) min ( -1 ) for acetate and MCA , respectively .
	manualset3
260003	7	426120	7	NULL	NULL	NULL	NULL	 23.1 nmol mg ( -1 ) min ( -1 )	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deh4p has apparent K ( m ) s of 5.5 and 8.9 muM and V ( max ) s of 9.1 and 23.1 nmol mg ( -1 ) min ( -1 ) for acetate and MCA , respectively .
	manualset3
260004	8	426120	7	NULL	NULL	NULL	NULL	acetate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deh4p has apparent K ( m ) s of 5.5 and 8.9 muM and V ( max ) s of 9.1 and 23.1 nmol mg ( -1 ) min ( -1 ) for acetate and MCA , respectively .
	manualset3
260006	9	426120	7	NULL	NULL	NULL	NULL	MCA	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deh4p has apparent K ( m ) s of 5.5 and 8.9 muM and V ( max ) s of 9.1 and 23.1 nmol mg ( -1 ) min ( -1 ) for acetate and MCA , respectively .
	manualset3
260009	1	426121	7	NULL	NULL	NULL	NULL	Dehydration	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dehydration due to hyperthermia induces both hyperosmolality and hypovolemia .
	manualset3
260010	2	426121	7	NULL	NULL	NULL	NULL	 hyperthermia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dehydration due to hyperthermia induces both hyperosmolality and hypovolemia .
	manualset3
260011	3	426121	7	NULL	NULL	NULL	NULL	hyperosmolality	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dehydration due to hyperthermia induces both hyperosmolality and hypovolemia .
	manualset3
260012	4	426121	7	NULL	NULL	NULL	NULL	hypovolemia	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dehydration due to hyperthermia induces both hyperosmolality and hypovolemia .
	manualset3
260014	1	426122	7	NULL	NULL	NULL	NULL	Dehydrocostuslactone 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dehydrocostuslactone exerted its antiproliferative effects by inducing cell cycle arrest and apoptosis .
	manualset3
260016	2	426122	7	NULL	NULL	NULL	NULL	antiproliferative effects	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dehydrocostuslactone exerted its antiproliferative effects by inducing cell cycle arrest and apoptosis .
	manualset3
260017	3	426122	7	NULL	NULL	NULL	NULL	cell cycle arrest 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dehydrocostuslactone exerted its antiproliferative effects by inducing cell cycle arrest and apoptosis .
	manualset3
260018	4	426122	7	NULL	NULL	NULL	NULL	apoptosis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dehydrocostuslactone exerted its antiproliferative effects by inducing cell cycle arrest and apoptosis .
	manualset3
260019	1	426123	7	NULL	NULL	NULL	NULL	Dehydroepiandrosterone ( DHA )	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dehydroepiandrosterone ( DHA ) , DHA sulfate ( DHAS ) , cortisol ( F ) , and androstenedione concentrations were determined in the medium by RIA .
	manualset3
260021	2	426123	7	NULL	NULL	NULL	NULL	DHA sulfate ( DHAS )	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dehydroepiandrosterone ( DHA ) , DHA sulfate ( DHAS ) , cortisol ( F ) , and androstenedione concentrations were determined in the medium by RIA .
	manualset3
260023	3	426123	7	NULL	NULL	NULL	NULL	cortisol ( F )	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dehydroepiandrosterone ( DHA ) , DHA sulfate ( DHAS ) , cortisol ( F ) , and androstenedione concentrations were determined in the medium by RIA .
	manualset3
260024	4	426123	7	NULL	NULL	NULL	NULL	androstenedione concentrations	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dehydroepiandrosterone ( DHA ) , DHA sulfate ( DHAS ) , cortisol ( F ) , and androstenedione concentrations were determined in the medium by RIA .
	manualset3
260025	5	426123	7	NULL	NULL	NULL	NULL	medium	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dehydroepiandrosterone ( DHA ) , DHA sulfate ( DHAS ) , cortisol ( F ) , and androstenedione concentrations were determined in the medium by RIA .
	manualset3
260026	6	426123	7	NULL	NULL	NULL	NULL	RIA	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dehydroepiandrosterone ( DHA ) , DHA sulfate ( DHAS ) , cortisol ( F ) , and androstenedione concentrations were determined in the medium by RIA .
	manualset3
260027	1	426124	7	NULL	NULL	NULL	NULL	Delayed carbon monoxide ( CO ) encephalopathy	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delayed carbon monoxide ( CO ) encephalopathy is a serious complication of acute CO poisoning .
	manualset3
260028	2	426124	7	NULL	NULL	NULL	NULL	serious complication	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delayed carbon monoxide ( CO ) encephalopathy is a serious complication of acute CO poisoning .
	manualset3
260029	3	426124	7	NULL	NULL	NULL	NULL	acute CO poisoning	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delayed carbon monoxide ( CO ) encephalopathy is a serious complication of acute CO poisoning .
	manualset3
260030	1	426125	7	NULL	NULL	NULL	NULL	Delayed pericardial tamponade	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delayed pericardial tamponade after penetrating chest trauma .
	manualset3
260031	2	426125	7	NULL	NULL	NULL	NULL	chest trauma	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delayed pericardial tamponade after penetrating chest trauma .
	manualset3
260206	1	426126	7	NULL	NULL	NULL	NULL	Deletion frequencies	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion frequencies of MST markers along the 12q12-q14 .3 locus suggest that the targeted gene of deletion is located within a 170-kb region bordered by the markers D12S1504 ( approximately 65 kb upstream of HMGA2 ) and D12S1509 ( in intron 3 of HMGA2 ) at the 12q14 .3 locus .
	manualset3
260207	2	426126	7	NULL	NULL	NULL	NULL	MST markers 	Chromosome												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion frequencies of MST markers along the 12q12-q14 .3 locus suggest that the targeted gene of deletion is located within a 170-kb region bordered by the markers D12S1504 ( approximately 65 kb upstream of HMGA2 ) and D12S1509 ( in intron 3 of HMGA2 ) at the 12q14 .3 locus .
	manualset3
260208	3	426126	7	NULL	NULL	NULL	NULL	12q12-q14 .3 locus	Chromosome												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion frequencies of MST markers along the 12q12-q14 .3 locus suggest that the targeted gene of deletion is located within a 170-kb region bordered by the markers D12S1504 ( approximately 65 kb upstream of HMGA2 ) and D12S1509 ( in intron 3 of HMGA2 ) at the 12q14 .3 locus .
	manualset3
260209	4	426126	7	NULL	NULL	NULL	NULL	 targeted gene of deletion	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion frequencies of MST markers along the 12q12-q14 .3 locus suggest that the targeted gene of deletion is located within a 170-kb region bordered by the markers D12S1504 ( approximately 65 kb upstream of HMGA2 ) and D12S1509 ( in intron 3 of HMGA2 ) at the 12q14 .3 locus .
	manualset3
260210	5	426126	7	NULL	NULL	NULL	NULL	 170-kb region	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion frequencies of MST markers along the 12q12-q14 .3 locus suggest that the targeted gene of deletion is located within a 170-kb region bordered by the markers D12S1504 ( approximately 65 kb upstream of HMGA2 ) and D12S1509 ( in intron 3 of HMGA2 ) at the 12q14 .3 locus .
	manualset3
260211	6	426126	7	NULL	NULL	NULL	NULL	markers D12S1504	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion frequencies of MST markers along the 12q12-q14 .3 locus suggest that the targeted gene of deletion is located within a 170-kb region bordered by the markers D12S1504 ( approximately 65 kb upstream of HMGA2 ) and D12S1509 ( in intron 3 of HMGA2 ) at the 12q14 .3 locus .
	manualset3
260212	7	426126	7	NULL	NULL	NULL	NULL	65 kb upstream	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion frequencies of MST markers along the 12q12-q14 .3 locus suggest that the targeted gene of deletion is located within a 170-kb region bordered by the markers D12S1504 ( approximately 65 kb upstream of HMGA2 ) and D12S1509 ( in intron 3 of HMGA2 ) at the 12q14 .3 locus .
	manualset3
260213	8	426126	7	NULL	NULL	NULL	NULL	 HMGA2 	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion frequencies of MST markers along the 12q12-q14 .3 locus suggest that the targeted gene of deletion is located within a 170-kb region bordered by the markers D12S1504 ( approximately 65 kb upstream of HMGA2 ) and D12S1509 ( in intron 3 of HMGA2 ) at the 12q14 .3 locus .
	manualset3
260214	9	426126	7	NULL	NULL	NULL	NULL	D12S1509	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion frequencies of MST markers along the 12q12-q14 .3 locus suggest that the targeted gene of deletion is located within a 170-kb region bordered by the markers D12S1504 ( approximately 65 kb upstream of HMGA2 ) and D12S1509 ( in intron 3 of HMGA2 ) at the 12q14 .3 locus .
	manualset3
260215	10	426126	7	NULL	NULL	NULL	NULL	 intron 3	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion frequencies of MST markers along the 12q12-q14 .3 locus suggest that the targeted gene of deletion is located within a 170-kb region bordered by the markers D12S1504 ( approximately 65 kb upstream of HMGA2 ) and D12S1509 ( in intron 3 of HMGA2 ) at the 12q14 .3 locus .
	manualset3
260216	11	426126	7	NULL	NULL	NULL	NULL	HMGA2	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion frequencies of MST markers along the 12q12-q14 .3 locus suggest that the targeted gene of deletion is located within a 170-kb region bordered by the markers D12S1504 ( approximately 65 kb upstream of HMGA2 ) and D12S1509 ( in intron 3 of HMGA2 ) at the 12q14 .3 locus .
	manualset3
260217	12	426126	7	NULL	NULL	NULL	NULL	12q14 .3 locus 	Chromosome												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion frequencies of MST markers along the 12q12-q14 .3 locus suggest that the targeted gene of deletion is located within a 170-kb region bordered by the markers D12S1504 ( approximately 65 kb upstream of HMGA2 ) and D12S1509 ( in intron 3 of HMGA2 ) at the 12q14 .3 locus .
	manualset3
260218	1	426127	7	NULL	NULL	NULL	NULL	Deletion	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of 11q23 is a frequent event in the evolution of MYCN single-copy high-risk neuroblastomas .
	manualset3
260219	2	426127	7	NULL	NULL	NULL	NULL	11q23	Chromosome												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of 11q23 is a frequent event in the evolution of MYCN single-copy high-risk neuroblastomas .
	manualset3
260220	3	426127	7	NULL	NULL	NULL	NULL	 frequent event	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of 11q23 is a frequent event in the evolution of MYCN single-copy high-risk neuroblastomas .
	manualset3
260221	4	426127	7	NULL	NULL	NULL	NULL	evolution 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of 11q23 is a frequent event in the evolution of MYCN single-copy high-risk neuroblastomas .
	manualset3
260222	5	426127	7	NULL	NULL	NULL	NULL	MYCN single-copy high-risk neuroblastomas	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of 11q23 is a frequent event in the evolution of MYCN single-copy high-risk neuroblastomas .
	manualset3
260223	1	426128	7	NULL	NULL	NULL	NULL	Deletion	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of five amino-acid residues from the C-terminus resulted in a complete loss of both enzymatic activity and formation of the cube-like structure , but the deletion of only the last two residues had no effect on either function , suggesting the important roles of the C-terminal leucine triplet ( Leu383-384-385 ) .
	manualset3
260224	2	426128	7	NULL	NULL	NULL	NULL	five amino-acid residues	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of five amino-acid residues from the C-terminus resulted in a complete loss of both enzymatic activity and formation of the cube-like structure , but the deletion of only the last two residues had no effect on either function , suggesting the important roles of the C-terminal leucine triplet ( Leu383-384-385 ) .
	manualset3
260225	3	426128	7	NULL	NULL	NULL	NULL	C-terminus	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of five amino-acid residues from the C-terminus resulted in a complete loss of both enzymatic activity and formation of the cube-like structure , but the deletion of only the last two residues had no effect on either function , suggesting the important roles of the C-terminal leucine triplet ( Leu383-384-385 ) .
	manualset3
260226	4	426128	7	NULL	NULL	NULL	NULL	complete loss	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of five amino-acid residues from the C-terminus resulted in a complete loss of both enzymatic activity and formation of the cube-like structure , but the deletion of only the last two residues had no effect on either function , suggesting the important roles of the C-terminal leucine triplet ( Leu383-384-385 ) .
	manualset3
260227	5	426128	7	NULL	NULL	NULL	NULL	enzymatic activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of five amino-acid residues from the C-terminus resulted in a complete loss of both enzymatic activity and formation of the cube-like structure , but the deletion of only the last two residues had no effect on either function , suggesting the important roles of the C-terminal leucine triplet ( Leu383-384-385 ) .
	manualset3
260228	6	426128	7	NULL	NULL	NULL	NULL	 formation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of five amino-acid residues from the C-terminus resulted in a complete loss of both enzymatic activity and formation of the cube-like structure , but the deletion of only the last two residues had no effect on either function , suggesting the important roles of the C-terminal leucine triplet ( Leu383-384-385 ) .
	manualset3
260229	7	426128	7	NULL	NULL	NULL	NULL	 cube-like structure	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of five amino-acid residues from the C-terminus resulted in a complete loss of both enzymatic activity and formation of the cube-like structure , but the deletion of only the last two residues had no effect on either function , suggesting the important roles of the C-terminal leucine triplet ( Leu383-384-385 ) .
	manualset3
260230	8	426128	7	NULL	NULL	NULL	NULL	deletion	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of five amino-acid residues from the C-terminus resulted in a complete loss of both enzymatic activity and formation of the cube-like structure , but the deletion of only the last two residues had no effect on either function , suggesting the important roles of the C-terminal leucine triplet ( Leu383-384-385 ) .
	manualset3
260231	9	426128	7	NULL	NULL	NULL	NULL	 last two residues	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of five amino-acid residues from the C-terminus resulted in a complete loss of both enzymatic activity and formation of the cube-like structure , but the deletion of only the last two residues had no effect on either function , suggesting the important roles of the C-terminal leucine triplet ( Leu383-384-385 ) .
	manualset3
260232	10	426128	7	NULL	NULL	NULL	NULL	function	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of five amino-acid residues from the C-terminus resulted in a complete loss of both enzymatic activity and formation of the cube-like structure , but the deletion of only the last two residues had no effect on either function , suggesting the important roles of the C-terminal leucine triplet ( Leu383-384-385 ) .
	manualset3
260233	11	426128	7	NULL	NULL	NULL	NULL	 important roles	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of five amino-acid residues from the C-terminus resulted in a complete loss of both enzymatic activity and formation of the cube-like structure , but the deletion of only the last two residues had no effect on either function , suggesting the important roles of the C-terminal leucine triplet ( Leu383-384-385 ) .
	manualset3
260234	12	426128	7	NULL	NULL	NULL	NULL	C-terminal leucine triplet ( Leu383-384-385 )	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of five amino-acid residues from the C-terminus resulted in a complete loss of both enzymatic activity and formation of the cube-like structure , but the deletion of only the last two residues had no effect on either function , suggesting the important roles of the C-terminal leucine triplet ( Leu383-384-385 ) .
	manualset3
260240	1	426129	7	NULL	NULL	NULL	NULL	Deletion	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of insulin or EGF from SFM resulted in cell growth similar to that of cells seeded in basal medium alone .
	manualset3
260242	2	426129	7	NULL	NULL	NULL	NULL	 insulin 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of insulin or EGF from SFM resulted in cell growth similar to that of cells seeded in basal medium alone .
	manualset3
260245	3	426129	7	NULL	NULL	NULL	NULL	EGF	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of insulin or EGF from SFM resulted in cell growth similar to that of cells seeded in basal medium alone .
	manualset3
260250	4	426129	7	NULL	NULL	NULL	NULL	 SFM	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of insulin or EGF from SFM resulted in cell growth similar to that of cells seeded in basal medium alone .
	manualset3
260252	5	426129	7	NULL	NULL	NULL	NULL	cell growth	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of insulin or EGF from SFM resulted in cell growth similar to that of cells seeded in basal medium alone .
	manualset3
260254	6	426129	7	NULL	NULL	NULL	NULL	 cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of insulin or EGF from SFM resulted in cell growth similar to that of cells seeded in basal medium alone .
	manualset3
260256	7	426129	7	NULL	NULL	NULL	NULL	basal medium	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of insulin or EGF from SFM resulted in cell growth similar to that of cells seeded in basal medium alone .
	manualset3
260267	1	426130	7	NULL	NULL	NULL	NULL	Deletion	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of the C terminus , which is not conserved among the members of this family , did not affect the binding capacity or the substrate specificity of the protein .
	manualset3
260269	2	426130	7	NULL	NULL	NULL	NULL	C terminus 	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of the C terminus , which is not conserved among the members of this family , did not affect the binding capacity or the substrate specificity of the protein .
	manualset3
260271	3	426130	7	NULL	NULL	NULL	NULL	members	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of the C terminus , which is not conserved among the members of this family , did not affect the binding capacity or the substrate specificity of the protein .
	manualset3
260272	4	426130	7	NULL	NULL	NULL	NULL	family	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of the C terminus , which is not conserved among the members of this family , did not affect the binding capacity or the substrate specificity of the protein .
	manualset3
260273	5	426130	7	NULL	NULL	NULL	NULL	binding capacity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of the C terminus , which is not conserved among the members of this family , did not affect the binding capacity or the substrate specificity of the protein .
	manualset3
260274	6	426130	7	NULL	NULL	NULL	NULL	substrate specificity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of the C terminus , which is not conserved among the members of this family , did not affect the binding capacity or the substrate specificity of the protein .
	manualset3
260275	7	426130	7	NULL	NULL	NULL	NULL	protein	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of the C terminus , which is not conserved among the members of this family , did not affect the binding capacity or the substrate specificity of the protein .
	manualset3
260278	1	426131	7	NULL	NULL	NULL	NULL	Deletion 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of the arcA gene caused about a 2-fold increase in the ptsG expression , and overexpression of ArcA significantly decreased glucose consumption .
	manualset3
260279	2	426131	7	NULL	NULL	NULL	NULL	 arcA gene 	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of the arcA gene caused about a 2-fold increase in the ptsG expression , and overexpression of ArcA significantly decreased glucose consumption .
	manualset3
260280	3	426131	7	NULL	NULL	NULL	NULL	2-fold increase	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of the arcA gene caused about a 2-fold increase in the ptsG expression , and overexpression of ArcA significantly decreased glucose consumption .
	manualset3
260281	4	426131	7	NULL	NULL	NULL	NULL	ptsG expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of the arcA gene caused about a 2-fold increase in the ptsG expression , and overexpression of ArcA significantly decreased glucose consumption .
	manualset3
260282	5	426131	7	NULL	NULL	NULL	NULL	overexpression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of the arcA gene caused about a 2-fold increase in the ptsG expression , and overexpression of ArcA significantly decreased glucose consumption .
	manualset3
260283	6	426131	7	NULL	NULL	NULL	NULL	ArcA	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of the arcA gene caused about a 2-fold increase in the ptsG expression , and overexpression of ArcA significantly decreased glucose consumption .
	manualset3
260285	7	426131	7	NULL	NULL	NULL	NULL	 glucose consumption	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletion of the arcA gene caused about a 2-fold increase in the ptsG expression , and overexpression of ArcA significantly decreased glucose consumption .
	manualset3
260521	1	426132	7	NULL	NULL	NULL	NULL	Deletions	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletions beginning from approximately +10 to +25 and extending further downstream reduced transcription to 20-40 % of wild type , whereas a deletion beginning at +31 had little or no effect .
	manualset3
260522	2	426132	7	NULL	NULL	NULL	NULL	 +10	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletions beginning from approximately +10 to +25 and extending further downstream reduced transcription to 20-40 % of wild type , whereas a deletion beginning at +31 had little or no effect .
	manualset3
260523	3	426132	7	NULL	NULL	NULL	NULL	+25	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletions beginning from approximately +10 to +25 and extending further downstream reduced transcription to 20-40 % of wild type , whereas a deletion beginning at +31 had little or no effect .
	manualset3
260524	4	426132	7	NULL	NULL	NULL	NULL	downstream 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletions beginning from approximately +10 to +25 and extending further downstream reduced transcription to 20-40 % of wild type , whereas a deletion beginning at +31 had little or no effect .
	manualset3
260525	5	426132	7	NULL	NULL	NULL	NULL	transcription	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletions beginning from approximately +10 to +25 and extending further downstream reduced transcription to 20-40 % of wild type , whereas a deletion beginning at +31 had little or no effect .
	manualset3
260526	6	426132	7	NULL	NULL	NULL	NULL	20-40 % 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletions beginning from approximately +10 to +25 and extending further downstream reduced transcription to 20-40 % of wild type , whereas a deletion beginning at +31 had little or no effect .
	manualset3
260527	7	426132	7	NULL	NULL	NULL	NULL	wild type	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletions beginning from approximately +10 to +25 and extending further downstream reduced transcription to 20-40 % of wild type , whereas a deletion beginning at +31 had little or no effect .
	manualset3
260528	8	426132	7	NULL	NULL	NULL	NULL	deletion 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletions beginning from approximately +10 to +25 and extending further downstream reduced transcription to 20-40 % of wild type , whereas a deletion beginning at +31 had little or no effect .
	manualset3
260529	9	426132	7	NULL	NULL	NULL	NULL	+31	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletions beginning from approximately +10 to +25 and extending further downstream reduced transcription to 20-40 % of wild type , whereas a deletion beginning at +31 had little or no effect .
	manualset3
260530	10	426132	7	NULL	NULL	NULL	NULL	effect	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletions beginning from approximately +10 to +25 and extending further downstream reduced transcription to 20-40 % of wild type , whereas a deletion beginning at +31 had little or no effect .
	manualset3
260531	1	426133	7	NULL	NULL	NULL	NULL	Deletions 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletions of the regions upstream of -946 bp and upstream of -684 bp caused a major decrease of GUS activity .
	manualset3
260532	2	426133	7	NULL	NULL	NULL	NULL	 regions 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletions of the regions upstream of -946 bp and upstream of -684 bp caused a major decrease of GUS activity .
	manualset3
260533	3	426133	7	NULL	NULL	NULL	NULL	 upstream	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletions of the regions upstream of -946 bp and upstream of -684 bp caused a major decrease of GUS activity .
	manualset3
260534	4	426133	7	NULL	NULL	NULL	NULL	-946 bp 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletions of the regions upstream of -946 bp and upstream of -684 bp caused a major decrease of GUS activity .
	manualset3
260535	5	426133	7	NULL	NULL	NULL	NULL	upstream	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletions of the regions upstream of -946 bp and upstream of -684 bp caused a major decrease of GUS activity .
	manualset3
260536	6	426133	7	NULL	NULL	NULL	NULL	 -684 bp	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletions of the regions upstream of -946 bp and upstream of -684 bp caused a major decrease of GUS activity .
	manualset3
260537	7	426133	7	NULL	NULL	NULL	NULL	major decrease	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletions of the regions upstream of -946 bp and upstream of -684 bp caused a major decrease of GUS activity .
	manualset3
260538	8	426133	7	NULL	NULL	NULL	NULL	GUS activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletions of the regions upstream of -946 bp and upstream of -684 bp caused a major decrease of GUS activity .
	manualset3
260539	1	426134	7	NULL	NULL	NULL	NULL	NEUROPATHIES	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( NEUROPATHIES OF BRONCHIAL CANCER ) .
	manualset3
260540	2	426134	7	NULL	NULL	NULL	NULL	BRONCHIAL CANCER	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( NEUROPATHIES OF BRONCHIAL CANCER ) .
	manualset3
260541	1	426135	7	NULL	NULL	NULL	NULL	Deletions	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletions of the transcription factor Ikaros in myeloproliferative neoplasms .
	manualset3
260542	2	426135	7	NULL	NULL	NULL	NULL	transcription factor Ikaros	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletions of the transcription factor Ikaros in myeloproliferative neoplasms .
	manualset3
260543	3	426135	7	NULL	NULL	NULL	NULL	myeloproliferative neoplasms	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletions of the transcription factor Ikaros in myeloproliferative neoplasms .
	manualset3
260544	1	426136	7	NULL	NULL	NULL	NULL	Deletions 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletions within the cysteine-rich region disrupt the interaction between dystrophin and the DAP complex , leading to a severe dystrophic pathology .
	manualset3
260545	2	426136	7	NULL	NULL	NULL	NULL	cysteine-rich region	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletions within the cysteine-rich region disrupt the interaction between dystrophin and the DAP complex , leading to a severe dystrophic pathology .
	manualset3
260546	3	426136	7	NULL	NULL	NULL	NULL	interaction 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletions within the cysteine-rich region disrupt the interaction between dystrophin and the DAP complex , leading to a severe dystrophic pathology .
	manualset3
260547	4	426136	7	NULL	NULL	NULL	NULL	dystrophin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletions within the cysteine-rich region disrupt the interaction between dystrophin and the DAP complex , leading to a severe dystrophic pathology .
	manualset3
260548	5	426136	7	NULL	NULL	NULL	NULL	DAP complex 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletions within the cysteine-rich region disrupt the interaction between dystrophin and the DAP complex , leading to a severe dystrophic pathology .
	manualset3
260549	6	426136	7	NULL	NULL	NULL	NULL	severe dystrophic pathology	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deletions within the cysteine-rich region disrupt the interaction between dystrophin and the DAP complex , leading to a severe dystrophic pathology .
	manualset3
260550	1	426137	7	NULL	NULL	NULL	NULL	Deliberate outbreaks	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deliberate and natural outbreaks of infectious disease , the prevalence of antibiotic resistant strains , and the ease by which antibiotic resistant bacteria can be intentionally engineered all underscore the necessity of effective vaccines and continued development of novel antimicrobial/antiviral therapeutics .
	manualset3
260551	2	426137	7	NULL	NULL	NULL	NULL	natural outbreaks	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deliberate and natural outbreaks of infectious disease , the prevalence of antibiotic resistant strains , and the ease by which antibiotic resistant bacteria can be intentionally engineered all underscore the necessity of effective vaccines and continued development of novel antimicrobial/antiviral therapeutics .
	manualset3
260552	3	426137	7	NULL	NULL	NULL	NULL	 infectious disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deliberate and natural outbreaks of infectious disease , the prevalence of antibiotic resistant strains , and the ease by which antibiotic resistant bacteria can be intentionally engineered all underscore the necessity of effective vaccines and continued development of novel antimicrobial/antiviral therapeutics .
	manualset3
260553	4	426137	7	NULL	NULL	NULL	NULL	prevalence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deliberate and natural outbreaks of infectious disease , the prevalence of antibiotic resistant strains , and the ease by which antibiotic resistant bacteria can be intentionally engineered all underscore the necessity of effective vaccines and continued development of novel antimicrobial/antiviral therapeutics .
	manualset3
260554	5	426137	7	NULL	NULL	NULL	NULL	antibiotic resistant strains	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deliberate and natural outbreaks of infectious disease , the prevalence of antibiotic resistant strains , and the ease by which antibiotic resistant bacteria can be intentionally engineered all underscore the necessity of effective vaccines and continued development of novel antimicrobial/antiviral therapeutics .
	manualset3
260555	6	426137	7	NULL	NULL	NULL	NULL	antibiotic resistant bacteria	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deliberate and natural outbreaks of infectious disease , the prevalence of antibiotic resistant strains , and the ease by which antibiotic resistant bacteria can be intentionally engineered all underscore the necessity of effective vaccines and continued development of novel antimicrobial/antiviral therapeutics .
	manualset3
260557	8	426137	7	NULL	NULL	NULL	NULL	 effective vaccines	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deliberate and natural outbreaks of infectious disease , the prevalence of antibiotic resistant strains , and the ease by which antibiotic resistant bacteria can be intentionally engineered all underscore the necessity of effective vaccines and continued development of novel antimicrobial/antiviral therapeutics .
	manualset3
260558	9	426137	7	NULL	NULL	NULL	NULL	continued development 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deliberate and natural outbreaks of infectious disease , the prevalence of antibiotic resistant strains , and the ease by which antibiotic resistant bacteria can be intentionally engineered all underscore the necessity of effective vaccines and continued development of novel antimicrobial/antiviral therapeutics .
	manualset3
260559	10	426137	7	NULL	NULL	NULL	NULL	novel antimicrobial/antiviral therapeutics 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deliberate and natural outbreaks of infectious disease , the prevalence of antibiotic resistant strains , and the ease by which antibiotic resistant bacteria can be intentionally engineered all underscore the necessity of effective vaccines and continued development of novel antimicrobial/antiviral therapeutics .
	manualset3
260560	1	426138	7	NULL	NULL	NULL	NULL	Delirium	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delirium , an acute confusional state with changes in attention and cognition , is a common cause of morbidity and mortality among hospitalized elders .
	manualset3
260561	2	426138	7	NULL	NULL	NULL	NULL	acute confusional state	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delirium , an acute confusional state with changes in attention and cognition , is a common cause of morbidity and mortality among hospitalized elders .
	manualset3
260562	3	426138	7	NULL	NULL	NULL	NULL	changes	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delirium , an acute confusional state with changes in attention and cognition , is a common cause of morbidity and mortality among hospitalized elders .
	manualset3
260563	4	426138	7	NULL	NULL	NULL	NULL	attention	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delirium , an acute confusional state with changes in attention and cognition , is a common cause of morbidity and mortality among hospitalized elders .
	manualset3
260564	5	426138	7	NULL	NULL	NULL	NULL	cognition	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delirium , an acute confusional state with changes in attention and cognition , is a common cause of morbidity and mortality among hospitalized elders .
	manualset3
260565	6	426138	7	NULL	NULL	NULL	NULL	 common cause 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delirium , an acute confusional state with changes in attention and cognition , is a common cause of morbidity and mortality among hospitalized elders .
	manualset3
260566	7	426138	7	NULL	NULL	NULL	NULL	 morbidity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delirium , an acute confusional state with changes in attention and cognition , is a common cause of morbidity and mortality among hospitalized elders .
	manualset3
260567	8	426138	7	NULL	NULL	NULL	NULL	mortality	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delirium , an acute confusional state with changes in attention and cognition , is a common cause of morbidity and mortality among hospitalized elders .
	manualset3
260568	9	426138	7	NULL	NULL	NULL	NULL	hospitalized elders 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delirium , an acute confusional state with changes in attention and cognition , is a common cause of morbidity and mortality among hospitalized elders .
	manualset3
260569	1	426139	7	NULL	NULL	NULL	NULL	Delivery	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delivery of NFs to the axon hillock inner plasma membrane surface , and their subsequent translocation into neurites , was also prevented by vinblastine-mediated inhibition of microtubule assembly .
	manualset3
260570	2	426139	7	NULL	NULL	NULL	NULL	NFs	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delivery of NFs to the axon hillock inner plasma membrane surface , and their subsequent translocation into neurites , was also prevented by vinblastine-mediated inhibition of microtubule assembly .
	manualset3
260571	3	426139	7	NULL	NULL	NULL	NULL	axon hillock inner plasma membrane surface	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delivery of NFs to the axon hillock inner plasma membrane surface , and their subsequent translocation into neurites , was also prevented by vinblastine-mediated inhibition of microtubule assembly .
	manualset3
260572	4	426139	7	NULL	NULL	NULL	NULL	translocation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delivery of NFs to the axon hillock inner plasma membrane surface , and their subsequent translocation into neurites , was also prevented by vinblastine-mediated inhibition of microtubule assembly .
	manualset3
260573	5	426139	7	NULL	NULL	NULL	NULL	neurites	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delivery of NFs to the axon hillock inner plasma membrane surface , and their subsequent translocation into neurites , was also prevented by vinblastine-mediated inhibition of microtubule assembly .
	manualset3
260574	6	426139	7	NULL	NULL	NULL	NULL	vinblastine-mediated inhibition	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delivery of NFs to the axon hillock inner plasma membrane surface , and their subsequent translocation into neurites , was also prevented by vinblastine-mediated inhibition of microtubule assembly .
	manualset3
260575	7	426139	7	NULL	NULL	NULL	NULL	microtubule assembly	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delivery of NFs to the axon hillock inner plasma membrane surface , and their subsequent translocation into neurites , was also prevented by vinblastine-mediated inhibition of microtubule assembly .
	manualset3
260576	1	426140	7	NULL	NULL	NULL	NULL	Delivery	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delivery of ofloxacin to the lung and alveolar macrophages via hyaluronan microspheres for the treatment of tuberculosis .
	manualset3
260577	2	426140	7	NULL	NULL	NULL	NULL	ofloxacin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delivery of ofloxacin to the lung and alveolar macrophages via hyaluronan microspheres for the treatment of tuberculosis .
	manualset3
260578	3	426140	7	NULL	NULL	NULL	NULL	 lung 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delivery of ofloxacin to the lung and alveolar macrophages via hyaluronan microspheres for the treatment of tuberculosis .
	manualset3
260579	4	426140	7	NULL	NULL	NULL	NULL	alveolar macrophages	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delivery of ofloxacin to the lung and alveolar macrophages via hyaluronan microspheres for the treatment of tuberculosis .
	manualset3
260580	5	426140	7	NULL	NULL	NULL	NULL	hyaluronan microspheres 	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delivery of ofloxacin to the lung and alveolar macrophages via hyaluronan microspheres for the treatment of tuberculosis .
	manualset3
260581	6	426140	7	NULL	NULL	NULL	NULL	treatment 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delivery of ofloxacin to the lung and alveolar macrophages via hyaluronan microspheres for the treatment of tuberculosis .
	manualset3
260582	7	426140	7	NULL	NULL	NULL	NULL	tuberculosis 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delivery of ofloxacin to the lung and alveolar macrophages via hyaluronan microspheres for the treatment of tuberculosis .
	manualset3
260583	1	426141	7	NULL	NULL	NULL	NULL	Delta-like ligand 4-Notch signaling 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delta-like ligand 4-Notch signaling regulates bone marrow-derived pericyte/vascular smooth muscle cell formation .
	manualset3
260584	2	426141	7	NULL	NULL	NULL	NULL	bone marrow-derived pericyte/vascular smooth muscle cell formation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delta-like ligand 4-Notch signaling regulates bone marrow-derived pericyte/vascular smooth muscle cell formation .
	manualset3
260585	1	426142	7	NULL	NULL	NULL	NULL	Delta-sleep-inducing peptide	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delta-sleep-inducing peptide stimulates melatonin , 5-methoxytryptophol and serotonin secretion from perifused rat pineal glands .
	manualset3
260586	2	426142	7	NULL	NULL	NULL	NULL	melatonin secretion	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delta-sleep-inducing peptide stimulates melatonin , 5-methoxytryptophol and serotonin secretion from perifused rat pineal glands .
	manualset3
260587	3	426142	7	NULL	NULL	NULL	NULL	5-methoxytryptophol secretion	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delta-sleep-inducing peptide stimulates melatonin , 5-methoxytryptophol and serotonin secretion from perifused rat pineal glands .
	manualset3
260588	4	426142	7	NULL	NULL	NULL	NULL	serotonin secretion	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delta-sleep-inducing peptide stimulates melatonin , 5-methoxytryptophol and serotonin secretion from perifused rat pineal glands .
	manualset3
260589	5	426142	7	NULL	NULL	NULL	NULL	 perifused rat pineal glands	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Delta-sleep-inducing peptide stimulates melatonin , 5-methoxytryptophol and serotonin secretion from perifused rat pineal glands .
	manualset3
260813	1	426143	7	NULL	NULL	NULL	NULL	Deltamethrin ( DLM ) 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deltamethrin ( DLM ) , ( ( S ) - alpha-cyano-d-phenoxybenzyl - ( 1R , 3 R ) - e - ( 2 , 2 dibromovinyl ) -2 , 2 - dimethylcyclo-propane-1-carboxylate ) , is a pyrethroid insecticide widely used in agriculture and households .
	manualset3
260814	2	426143	7	NULL	NULL	NULL	NULL	 ( ( S ) - alpha-cyano-d-phenoxybenzyl - ( 1R , 3 R ) - e - ( 2 , 2 dibromovinyl ) -2 , 2 - dimethylcyclo-propane-1-carboxylate )	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deltamethrin ( DLM ) , ( ( S ) - alpha-cyano-d-phenoxybenzyl - ( 1R , 3 R ) - e - ( 2 , 2 dibromovinyl ) -2 , 2 - dimethylcyclo-propane-1-carboxylate ) , is a pyrethroid insecticide widely used in agriculture and households .
	manualset3
260816	3	426143	7	NULL	NULL	NULL	NULL	pyrethroid insecticide	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deltamethrin ( DLM ) , ( ( S ) - alpha-cyano-d-phenoxybenzyl - ( 1R , 3 R ) - e - ( 2 , 2 dibromovinyl ) -2 , 2 - dimethylcyclo-propane-1-carboxylate ) , is a pyrethroid insecticide widely used in agriculture and households .
	manualset3
260818	4	426143	7	NULL	NULL	NULL	NULL	agriculture	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deltamethrin ( DLM ) , ( ( S ) - alpha-cyano-d-phenoxybenzyl - ( 1R , 3 R ) - e - ( 2 , 2 dibromovinyl ) -2 , 2 - dimethylcyclo-propane-1-carboxylate ) , is a pyrethroid insecticide widely used in agriculture and households .
	manualset3
260819	5	426143	7	NULL	NULL	NULL	NULL	 households	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deltamethrin ( DLM ) , ( ( S ) - alpha-cyano-d-phenoxybenzyl - ( 1R , 3 R ) - e - ( 2 , 2 dibromovinyl ) -2 , 2 - dimethylcyclo-propane-1-carboxylate ) , is a pyrethroid insecticide widely used in agriculture and households .
	manualset3
260823	1	426144	7	NULL	NULL	NULL	NULL	experiential professional membership	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Demographic , educational , experiential professional membership , and school assignment variables were explored .
	manualset3
260825	2	426144	7	NULL	NULL	NULL	NULL	school assignment variables	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Demographic , educational , experiential professional membership , and school assignment variables were explored .
	manualset3
260831	1	426145	7	NULL	NULL	NULL	NULL	National Congress	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( National Congress in the diagnosis and treatment of upper digestive tract bleeding ) .
	manualset3
260832	2	426145	7	NULL	NULL	NULL	NULL	diagnosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( National Congress in the diagnosis and treatment of upper digestive tract bleeding ) .
	manualset3
260833	3	426145	7	NULL	NULL	NULL	NULL	treatment 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( National Congress in the diagnosis and treatment of upper digestive tract bleeding ) .
	manualset3
260834	4	426145	7	NULL	NULL	NULL	NULL	upper digestive tract bleeding	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( National Congress in the diagnosis and treatment of upper digestive tract bleeding ) .
	manualset3
260839	1	426146	7	NULL	NULL	NULL	NULL	Demonstration	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Demonstration of a direct carcinogenic effect of estradiol on Leydig cells of the mouse .
	manualset3
260840	2	426146	7	NULL	NULL	NULL	NULL	direct carcinogenic effect	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Demonstration of a direct carcinogenic effect of estradiol on Leydig cells of the mouse .
	manualset3
260842	3	426146	7	NULL	NULL	NULL	NULL	estradiol	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Demonstration of a direct carcinogenic effect of estradiol on Leydig cells of the mouse .
	manualset3
260844	4	426146	7	NULL	NULL	NULL	NULL	Leydig cells 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Demonstration of a direct carcinogenic effect of estradiol on Leydig cells of the mouse .
	manualset3
260846	5	426146	7	NULL	NULL	NULL	NULL	mouse	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Demonstration of a direct carcinogenic effect of estradiol on Leydig cells of the mouse .
	manualset3
260848	1	426147	7	NULL	NULL	NULL	NULL	Demonstration	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Demonstration of a growth factor encoded by a DNA virus is unprecedented and may expand our understanding of DNA virus-host interactions .
	manualset3
260849	2	426147	7	NULL	NULL	NULL	NULL	growth factor	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Demonstration of a growth factor encoded by a DNA virus is unprecedented and may expand our understanding of DNA virus-host interactions .
	manualset3
260851	3	426147	7	NULL	NULL	NULL	NULL	DNA virus	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Demonstration of a growth factor encoded by a DNA virus is unprecedented and may expand our understanding of DNA virus-host interactions .
	manualset3
260852	4	426147	7	NULL	NULL	NULL	NULL	understanding 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Demonstration of a growth factor encoded by a DNA virus is unprecedented and may expand our understanding of DNA virus-host interactions .
	manualset3
260854	5	426147	7	NULL	NULL	NULL	NULL	DNA virus-host interactions	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Demonstration of a growth factor encoded by a DNA virus is unprecedented and may expand our understanding of DNA virus-host interactions .
	manualset3
260857	1	426148	7	NULL	NULL	NULL	NULL	Dendriform pulmonary ossification	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dendriform pulmonary ossification , defined as `` widespread heterotopic bone formation within the lungs , '' is a rare entity , which is usually diagnosed upon postmortem examination .
	manualset3
260858	2	426148	7	NULL	NULL	NULL	NULL	 widespread heterotopic bone formation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dendriform pulmonary ossification , defined as `` widespread heterotopic bone formation within the lungs , '' is a rare entity , which is usually diagnosed upon postmortem examination .
	manualset3
260859	3	426148	7	NULL	NULL	NULL	NULL	 lungs	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dendriform pulmonary ossification , defined as `` widespread heterotopic bone formation within the lungs , '' is a rare entity , which is usually diagnosed upon postmortem examination .
	manualset3
260860	4	426148	7	NULL	NULL	NULL	NULL	postmortem examination	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dendriform pulmonary ossification , defined as `` widespread heterotopic bone formation within the lungs , '' is a rare entity , which is usually diagnosed upon postmortem examination .
	manualset3
260861	5	426148	7	NULL	NULL	NULL	NULL	 rare entity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dendriform pulmonary ossification , defined as `` widespread heterotopic bone formation within the lungs , '' is a rare entity , which is usually diagnosed upon postmortem examination .
	manualset3
260862	1	426149	7	NULL	NULL	NULL	NULL	Dendritic cells ( DC )	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dendritic cells ( DC ) mediate airway Ag presentation and play key roles in asthma and infections .
	manualset3
260863	2	426149	7	NULL	NULL	NULL	NULL	airway Ag presentation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dendritic cells ( DC ) mediate airway Ag presentation and play key roles in asthma and infections .
	manualset3
260864	3	426149	7	NULL	NULL	NULL	NULL	key roles 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dendritic cells ( DC ) mediate airway Ag presentation and play key roles in asthma and infections .
	manualset3
260865	4	426149	7	NULL	NULL	NULL	NULL	asthma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dendritic cells ( DC ) mediate airway Ag presentation and play key roles in asthma and infections .
	manualset3
260866	5	426149	7	NULL	NULL	NULL	NULL	infections	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dendritic cells ( DC ) mediate airway Ag presentation and play key roles in asthma and infections .
	manualset3
260867	1	426150	7	NULL	NULL	NULL	NULL	Dendritic cells ( DCs ) 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dendritic cells ( DCs ) are key players in both initiating immunity ( immunogenic DCs ) and regulating immune responses ( tolerogenic DCs = tolDCs ) and are potential targets for the treatment of MS. While the immunogenic potential of DCs in fighting infection and cancer has been well established , approaches that exploit their tolerogenic features to promote transplantation tolerance and autoimmunity have emerged only more recently .
	manualset3
260868	2	426150	7	NULL	NULL	NULL	NULL	immunity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dendritic cells ( DCs ) are key players in both initiating immunity ( immunogenic DCs ) and regulating immune responses ( tolerogenic DCs = tolDCs ) and are potential targets for the treatment of MS. While the immunogenic potential of DCs in fighting infection and cancer has been well established , approaches that exploit their tolerogenic features to promote transplantation tolerance and autoimmunity have emerged only more recently .
	manualset3
260869	3	426150	7	NULL	NULL	NULL	NULL	immunogenic DCs 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dendritic cells ( DCs ) are key players in both initiating immunity ( immunogenic DCs ) and regulating immune responses ( tolerogenic DCs = tolDCs ) and are potential targets for the treatment of MS. While the immunogenic potential of DCs in fighting infection and cancer has been well established , approaches that exploit their tolerogenic features to promote transplantation tolerance and autoimmunity have emerged only more recently .
	manualset3
260870	4	426150	7	NULL	NULL	NULL	NULL	 key players	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dendritic cells ( DCs ) are key players in both initiating immunity ( immunogenic DCs ) and regulating immune responses ( tolerogenic DCs = tolDCs ) and are potential targets for the treatment of MS. While the immunogenic potential of DCs in fighting infection and cancer has been well established , approaches that exploit their tolerogenic features to promote transplantation tolerance and autoimmunity have emerged only more recently .
	manualset3
260871	5	426150	7	NULL	NULL	NULL	NULL	immune responses	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dendritic cells ( DCs ) are key players in both initiating immunity ( immunogenic DCs ) and regulating immune responses ( tolerogenic DCs = tolDCs ) and are potential targets for the treatment of MS. While the immunogenic potential of DCs in fighting infection and cancer has been well established , approaches that exploit their tolerogenic features to promote transplantation tolerance and autoimmunity have emerged only more recently .
	manualset3
260872	6	426150	7	NULL	NULL	NULL	NULL	tolerogenic DCs = tolDCs	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dendritic cells ( DCs ) are key players in both initiating immunity ( immunogenic DCs ) and regulating immune responses ( tolerogenic DCs = tolDCs ) and are potential targets for the treatment of MS. While the immunogenic potential of DCs in fighting infection and cancer has been well established , approaches that exploit their tolerogenic features to promote transplantation tolerance and autoimmunity have emerged only more recently .
	manualset3
260873	7	426150	7	NULL	NULL	NULL	NULL	 potential targets	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dendritic cells ( DCs ) are key players in both initiating immunity ( immunogenic DCs ) and regulating immune responses ( tolerogenic DCs = tolDCs ) and are potential targets for the treatment of MS. While the immunogenic potential of DCs in fighting infection and cancer has been well established , approaches that exploit their tolerogenic features to promote transplantation tolerance and autoimmunity have emerged only more recently .
	manualset3
260874	8	426150	7	NULL	NULL	NULL	NULL	treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dendritic cells ( DCs ) are key players in both initiating immunity ( immunogenic DCs ) and regulating immune responses ( tolerogenic DCs = tolDCs ) and are potential targets for the treatment of MS. While the immunogenic potential of DCs in fighting infection and cancer has been well established , approaches that exploit their tolerogenic features to promote transplantation tolerance and autoimmunity have emerged only more recently .
	manualset3
260875	9	426150	7	NULL	NULL	NULL	NULL	immunogenic potential	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dendritic cells ( DCs ) are key players in both initiating immunity ( immunogenic DCs ) and regulating immune responses ( tolerogenic DCs = tolDCs ) and are potential targets for the treatment of MS. While the immunogenic potential of DCs in fighting infection and cancer has been well established , approaches that exploit their tolerogenic features to promote transplantation tolerance and autoimmunity have emerged only more recently .
	manualset3
260876	10	426150	7	NULL	NULL	NULL	NULL	DCs	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dendritic cells ( DCs ) are key players in both initiating immunity ( immunogenic DCs ) and regulating immune responses ( tolerogenic DCs = tolDCs ) and are potential targets for the treatment of MS. While the immunogenic potential of DCs in fighting infection and cancer has been well established , approaches that exploit their tolerogenic features to promote transplantation tolerance and autoimmunity have emerged only more recently .
	manualset3
260877	11	426150	7	NULL	NULL	NULL	NULL	 infection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dendritic cells ( DCs ) are key players in both initiating immunity ( immunogenic DCs ) and regulating immune responses ( tolerogenic DCs = tolDCs ) and are potential targets for the treatment of MS. While the immunogenic potential of DCs in fighting infection and cancer has been well established , approaches that exploit their tolerogenic features to promote transplantation tolerance and autoimmunity have emerged only more recently .
	manualset3
260878	12	426150	7	NULL	NULL	NULL	NULL	cancer	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dendritic cells ( DCs ) are key players in both initiating immunity ( immunogenic DCs ) and regulating immune responses ( tolerogenic DCs = tolDCs ) and are potential targets for the treatment of MS. While the immunogenic potential of DCs in fighting infection and cancer has been well established , approaches that exploit their tolerogenic features to promote transplantation tolerance and autoimmunity have emerged only more recently .
	manualset3
260879	13	426150	7	NULL	NULL	NULL	NULL	tolerogenic features	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dendritic cells ( DCs ) are key players in both initiating immunity ( immunogenic DCs ) and regulating immune responses ( tolerogenic DCs = tolDCs ) and are potential targets for the treatment of MS. While the immunogenic potential of DCs in fighting infection and cancer has been well established , approaches that exploit their tolerogenic features to promote transplantation tolerance and autoimmunity have emerged only more recently .
	manualset3
260880	14	426150	7	NULL	NULL	NULL	NULL	transplantation tolerance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dendritic cells ( DCs ) are key players in both initiating immunity ( immunogenic DCs ) and regulating immune responses ( tolerogenic DCs = tolDCs ) and are potential targets for the treatment of MS. While the immunogenic potential of DCs in fighting infection and cancer has been well established , approaches that exploit their tolerogenic features to promote transplantation tolerance and autoimmunity have emerged only more recently .
	manualset3
260881	15	426150	7	NULL	NULL	NULL	NULL	autoimmunity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dendritic cells ( DCs ) are key players in both initiating immunity ( immunogenic DCs ) and regulating immune responses ( tolerogenic DCs = tolDCs ) and are potential targets for the treatment of MS. While the immunogenic potential of DCs in fighting infection and cancer has been well established , approaches that exploit their tolerogenic features to promote transplantation tolerance and autoimmunity have emerged only more recently .
	manualset3
264811	16	426150	7	NULL	NULL	NULL	NULL	MS	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dendritic cells ( DCs ) are key players in both initiating immunity ( immunogenic DCs ) and regulating immune responses ( tolerogenic DCs = tolDCs ) and are potential targets for the treatment of MS. While the immunogenic potential of DCs in fighting infection and cancer has been well established , approaches that exploit their tolerogenic features to promote transplantation tolerance and autoimmunity have emerged only more recently .
	manualset3
261118	1	426151	7	NULL	NULL	NULL	NULL	Dengue 1	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dengue 1 was the predominant virus until December 1981 , when dengue 4 became dominant .
	manualset3
261119	2	426151	7	NULL	NULL	NULL	NULL	virus 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dengue 1 was the predominant virus until December 1981 , when dengue 4 became dominant .
	manualset3
261124	3	426151	7	NULL	NULL	NULL	NULL	December 1981	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dengue 1 was the predominant virus until December 1981 , when dengue 4 became dominant .
	manualset3
261125	4	426151	7	NULL	NULL	NULL	NULL	dengue 4 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dengue 1 was the predominant virus until December 1981 , when dengue 4 became dominant .
	manualset3
261139	1	426152	7	NULL	NULL	NULL	NULL	Densely stacked multilamellar vesicles	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Densely stacked multilamellar and oligovesicular vesicles , bilayer cylinders , and tubes joining with vesicles of a salt-free catanionic extractant and surfactant system .
	manualset3
261140	2	426152	7	NULL	NULL	NULL	NULL	oligovesicular vesicles	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Densely stacked multilamellar and oligovesicular vesicles , bilayer cylinders , and tubes joining with vesicles of a salt-free catanionic extractant and surfactant system .
	manualset3
261141	3	426152	7	NULL	NULL	NULL	NULL	bilayer cylinders	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Densely stacked multilamellar and oligovesicular vesicles , bilayer cylinders , and tubes joining with vesicles of a salt-free catanionic extractant and surfactant system .
	manualset3
261142	4	426152	7	NULL	NULL	NULL	NULL	tubes	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Densely stacked multilamellar and oligovesicular vesicles , bilayer cylinders , and tubes joining with vesicles of a salt-free catanionic extractant and surfactant system .
	manualset3
261143	5	426152	7	NULL	NULL	NULL	NULL	 vesicles	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Densely stacked multilamellar and oligovesicular vesicles , bilayer cylinders , and tubes joining with vesicles of a salt-free catanionic extractant and surfactant system .
	manualset3
261144	6	426152	7	NULL	NULL	NULL	NULL	salt-free catanionic extractant 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Densely stacked multilamellar and oligovesicular vesicles , bilayer cylinders , and tubes joining with vesicles of a salt-free catanionic extractant and surfactant system .
	manualset3
261145	7	426152	7	NULL	NULL	NULL	NULL	surfactant system	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Densely stacked multilamellar and oligovesicular vesicles , bilayer cylinders , and tubes joining with vesicles of a salt-free catanionic extractant and surfactant system .
	manualset3
261146	1	426153	7	NULL	NULL	NULL	NULL	Densities	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Densities , heats of formation , detonation pressures and velocities , and specific impulses were calculated .
	manualset3
261147	2	426153	7	NULL	NULL	NULL	NULL	heats of formation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Densities , heats of formation , detonation pressures and velocities , and specific impulses were calculated .
	manualset3
261148	3	426153	7	NULL	NULL	NULL	NULL	detonation pressures	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Densities , heats of formation , detonation pressures and velocities , and specific impulses were calculated .
	manualset3
261149	4	426153	7	NULL	NULL	NULL	NULL	 velocities 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Densities , heats of formation , detonation pressures and velocities , and specific impulses were calculated .
	manualset3
261151	5	426153	7	NULL	NULL	NULL	NULL	specific impulses 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Densities , heats of formation , detonation pressures and velocities , and specific impulses were calculated .
	manualset3
261152	1	426154	7	NULL	NULL	NULL	NULL	Density functional theory ( DFT ) calculations	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Density functional theory ( DFT ) calculations at the B3LYP/6 -31 G ( d , p ) level of theory were used to optimize the molecular structure and the geometry was best reproduced by optimization of two interacting molecules .
	manualset3
261153	2	426154	7	NULL	NULL	NULL	NULL	B3LYP/6 -31 G ( d , p ) level	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Density functional theory ( DFT ) calculations at the B3LYP/6 -31 G ( d , p ) level of theory were used to optimize the molecular structure and the geometry was best reproduced by optimization of two interacting molecules .
	manualset3
261159	3	426154	7	NULL	NULL	NULL	NULL	theory	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Density functional theory ( DFT ) calculations at the B3LYP/6 -31 G ( d , p ) level of theory were used to optimize the molecular structure and the geometry was best reproduced by optimization of two interacting molecules .
	manualset3
261160	4	426154	7	NULL	NULL	NULL	NULL	molecular structure	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Density functional theory ( DFT ) calculations at the B3LYP/6 -31 G ( d , p ) level of theory were used to optimize the molecular structure and the geometry was best reproduced by optimization of two interacting molecules .
	manualset3
261161	5	426154	7	NULL	NULL	NULL	NULL	geometry	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Density functional theory ( DFT ) calculations at the B3LYP/6 -31 G ( d , p ) level of theory were used to optimize the molecular structure and the geometry was best reproduced by optimization of two interacting molecules .
	manualset3
261162	6	426154	7	NULL	NULL	NULL	NULL	optimization	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Density functional theory ( DFT ) calculations at the B3LYP/6 -31 G ( d , p ) level of theory were used to optimize the molecular structure and the geometry was best reproduced by optimization of two interacting molecules .
	manualset3
261163	7	426154	7	NULL	NULL	NULL	NULL	two interacting molecules	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Density functional theory ( DFT ) calculations at the B3LYP/6 -31 G ( d , p ) level of theory were used to optimize the molecular structure and the geometry was best reproduced by optimization of two interacting molecules .
	manualset3
261164	1	426155	7	NULL	NULL	NULL	NULL	Dental care	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dental care for the underserved children of Monterey County : meeting the challenge .
	manualset3
261165	2	426155	7	NULL	NULL	NULL	NULL	underserved children	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dental care for the underserved children of Monterey County : meeting the challenge .
	manualset3
261166	3	426155	7	NULL	NULL	NULL	NULL	Monterey County 	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dental care for the underserved children of Monterey County : meeting the challenge .
	manualset3
261167	4	426155	7	NULL	NULL	NULL	NULL	meeting	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dental care for the underserved children of Monterey County : meeting the challenge .
	manualset3
261168	5	426155	7	NULL	NULL	NULL	NULL	challenge	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dental care for the underserved children of Monterey County : meeting the challenge .
	manualset3
261169	1	426156	7	NULL	NULL	NULL	NULL	Dental caries	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dental caries was recorded according to WHO criteria .
	manualset3
261170	2	426156	7	NULL	NULL	NULL	NULL	WHO criteria	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dental caries was recorded according to WHO criteria .
	manualset3
261171	1	426157	7	NULL	NULL	NULL	NULL	Dental management 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dental management of patients with end-stage liver disease .
	manualset3
261172	2	426157	7	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dental management of patients with end-stage liver disease .
	manualset3
261173	3	426157	7	NULL	NULL	NULL	NULL	end-stage liver disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dental management of patients with end-stage liver disease .
	manualset3
261174	1	426158	7	NULL	NULL	NULL	NULL	Dental mercury amalgam	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dental mercury amalgam : Part III .
	manualset3
261175	2	426158	7	NULL	NULL	NULL	NULL	Part III	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dental mercury amalgam : Part III .
	manualset3
261176	1	426159	7	NULL	NULL	NULL	NULL	Dental pulp collagenase 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dental pulp collagenase : initial demonstration and characterization .
	manualset3
261177	2	426159	7	NULL	NULL	NULL	NULL	initial demonstration	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dental pulp collagenase : initial demonstration and characterization .
	manualset3
261178	3	426159	7	NULL	NULL	NULL	NULL	characterization	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dental pulp collagenase : initial demonstration and characterization .
	manualset3
261179	1	426160	7	NULL	NULL	NULL	NULL	Dental student development	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dental student development of cultural competence and social responsibility is recognized by educators as an important element in the overall shaping of minds and attitudes of modem dental practitioners .
	manualset3
261180	2	426160	7	NULL	NULL	NULL	NULL	cultural competence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dental student development of cultural competence and social responsibility is recognized by educators as an important element in the overall shaping of minds and attitudes of modem dental practitioners .
	manualset3
261181	3	426160	7	NULL	NULL	NULL	NULL	social responsibility	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dental student development of cultural competence and social responsibility is recognized by educators as an important element in the overall shaping of minds and attitudes of modem dental practitioners .
	manualset3
261182	4	426160	7	NULL	NULL	NULL	NULL	educators	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dental student development of cultural competence and social responsibility is recognized by educators as an important element in the overall shaping of minds and attitudes of modem dental practitioners .
	manualset3
261183	5	426160	7	NULL	NULL	NULL	NULL	 important element 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dental student development of cultural competence and social responsibility is recognized by educators as an important element in the overall shaping of minds and attitudes of modem dental practitioners .
	manualset3
261184	6	426160	7	NULL	NULL	NULL	NULL	overall shaping	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dental student development of cultural competence and social responsibility is recognized by educators as an important element in the overall shaping of minds and attitudes of modem dental practitioners .
	manualset3
261185	7	426160	7	NULL	NULL	NULL	NULL	minds 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dental student development of cultural competence and social responsibility is recognized by educators as an important element in the overall shaping of minds and attitudes of modem dental practitioners .
	manualset3
261186	8	426160	7	NULL	NULL	NULL	NULL	attitudes	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dental student development of cultural competence and social responsibility is recognized by educators as an important element in the overall shaping of minds and attitudes of modem dental practitioners .
	manualset3
261187	9	426160	7	NULL	NULL	NULL	NULL	modem dental practitioners	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dental student development of cultural competence and social responsibility is recognized by educators as an important element in the overall shaping of minds and attitudes of modem dental practitioners .
	manualset3
261188	1	426161	7	NULL	NULL	NULL	NULL	versatile suitable roentgen room 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( A versatile suitable roentgen room with a mobile BV-FS-system ) .
	manualset3
261189	2	426161	7	NULL	NULL	NULL	NULL	mobile BV-FS-system 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( A versatile suitable roentgen room with a mobile BV-FS-system ) .
	manualset3
261191	1	426162	7	NULL	NULL	NULL	NULL	Neoplastic pathology	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Neoplastic pathology of the vulva : unusual case of neurinoma of the clitoris ) .
	manualset3
261192	2	426162	7	NULL	NULL	NULL	NULL	 vulva 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Neoplastic pathology of the vulva : unusual case of neurinoma of the clitoris ) .
	manualset3
261193	3	426162	7	NULL	NULL	NULL	NULL	 unusual case	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Neoplastic pathology of the vulva : unusual case of neurinoma of the clitoris ) .
	manualset3
261194	4	426162	7	NULL	NULL	NULL	NULL	neurinoma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Neoplastic pathology of the vulva : unusual case of neurinoma of the clitoris ) .
	manualset3
261195	5	426162	7	NULL	NULL	NULL	NULL	clitoris	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Neoplastic pathology of the vulva : unusual case of neurinoma of the clitoris ) .
	manualset3
261197	1	426163	7	NULL	NULL	NULL	NULL	Dentistry 's leaders voice healthcare	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dentistry 's leaders voice healthcare reform concerns .
	manualset3
261198	2	426163	7	NULL	NULL	NULL	NULL	concerns	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dentistry 's leaders voice healthcare reform concerns .
	manualset3
261199	1	426164	7	NULL	NULL	NULL	NULL	Denture stomatitis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Denture stomatitis : a review .
	manualset3
261200	2	426164	7	NULL	NULL	NULL	NULL	review 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Denture stomatitis : a review .
	manualset3
261202	1	426165	7	NULL	NULL	NULL	NULL	Deoxyribonucleic acid	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deoxyribonucleic acid from 28 primary gastric adenocarcinomas were analyzed for point mutations in codons 12 , 13 , and 61 of the Ha-ras , Ki-ras , and N-ras protooncogenes using polymerase-catalyzed chain reaction methodology .
	manualset3
261203	2	426165	7	NULL	NULL	NULL	NULL	28 primary gastric adenocarcinomas	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deoxyribonucleic acid from 28 primary gastric adenocarcinomas were analyzed for point mutations in codons 12 , 13 , and 61 of the Ha-ras , Ki-ras , and N-ras protooncogenes using polymerase-catalyzed chain reaction methodology .
	manualset3
261204	3	426165	7	NULL	NULL	NULL	NULL	 point mutations	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deoxyribonucleic acid from 28 primary gastric adenocarcinomas were analyzed for point mutations in codons 12 , 13 , and 61 of the Ha-ras , Ki-ras , and N-ras protooncogenes using polymerase-catalyzed chain reaction methodology .
	manualset3
261205	4	426165	7	NULL	NULL	NULL	NULL	codons 12	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deoxyribonucleic acid from 28 primary gastric adenocarcinomas were analyzed for point mutations in codons 12 , 13 , and 61 of the Ha-ras , Ki-ras , and N-ras protooncogenes using polymerase-catalyzed chain reaction methodology .
	manualset3
261206	5	426165	7	NULL	NULL	NULL	NULL	codons 13	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deoxyribonucleic acid from 28 primary gastric adenocarcinomas were analyzed for point mutations in codons 12 , 13 , and 61 of the Ha-ras , Ki-ras , and N-ras protooncogenes using polymerase-catalyzed chain reaction methodology .
	manualset3
261207	6	426165	7	NULL	NULL	NULL	NULL	codons 61	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deoxyribonucleic acid from 28 primary gastric adenocarcinomas were analyzed for point mutations in codons 12 , 13 , and 61 of the Ha-ras , Ki-ras , and N-ras protooncogenes using polymerase-catalyzed chain reaction methodology .
	manualset3
261208	7	426165	7	NULL	NULL	NULL	NULL	Ha-ras	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deoxyribonucleic acid from 28 primary gastric adenocarcinomas were analyzed for point mutations in codons 12 , 13 , and 61 of the Ha-ras , Ki-ras , and N-ras protooncogenes using polymerase-catalyzed chain reaction methodology .
	manualset3
261209	8	426165	7	NULL	NULL	NULL	NULL	Ki-ras	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deoxyribonucleic acid from 28 primary gastric adenocarcinomas were analyzed for point mutations in codons 12 , 13 , and 61 of the Ha-ras , Ki-ras , and N-ras protooncogenes using polymerase-catalyzed chain reaction methodology .
	manualset3
261210	9	426165	7	NULL	NULL	NULL	NULL	N-ras protooncogenes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deoxyribonucleic acid from 28 primary gastric adenocarcinomas were analyzed for point mutations in codons 12 , 13 , and 61 of the Ha-ras , Ki-ras , and N-ras protooncogenes using polymerase-catalyzed chain reaction methodology .
	manualset3
261211	10	426165	7	NULL	NULL	NULL	NULL	polymerase-catalyzed chain reaction methodology	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deoxyribonucleic acid from 28 primary gastric adenocarcinomas were analyzed for point mutations in codons 12 , 13 , and 61 of the Ha-ras , Ki-ras , and N-ras protooncogenes using polymerase-catalyzed chain reaction methodology .
	manualset3
261212	1	426166	7	NULL	NULL	NULL	NULL	Dependence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dependence of somatic-fitness traits on regional factors increased with age .
	manualset3
261213	2	426166	7	NULL	NULL	NULL	NULL	somatic-fitness traits	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dependence of somatic-fitness traits on regional factors increased with age .
	manualset3
261214	3	426166	7	NULL	NULL	NULL	NULL	 regional factors	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dependence of somatic-fitness traits on regional factors increased with age .
	manualset3
261215	4	426166	7	NULL	NULL	NULL	NULL	age	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dependence of somatic-fitness traits on regional factors increased with age .
	manualset3
261216	1	426167	7	NULL	NULL	NULL	NULL	Ca2 +	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dependence on Ca2 + and tropomyosin of the actin-activated ATPase activity of phosphorylated gizzard myosin in the presence of low concentrations of Mg2 + .
	manualset3
261217	2	426167	7	NULL	NULL	NULL	NULL	tropomyosin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dependence on Ca2 + and tropomyosin of the actin-activated ATPase activity of phosphorylated gizzard myosin in the presence of low concentrations of Mg2 + .
	manualset3
261218	3	426167	7	NULL	NULL	NULL	NULL	actin-activated ATPase activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dependence on Ca2 + and tropomyosin of the actin-activated ATPase activity of phosphorylated gizzard myosin in the presence of low concentrations of Mg2 + .
	manualset3
261219	4	426167	7	NULL	NULL	NULL	NULL	phosphorylated gizzard myosin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dependence on Ca2 + and tropomyosin of the actin-activated ATPase activity of phosphorylated gizzard myosin in the presence of low concentrations of Mg2 + .
	manualset3
261220	5	426167	7	NULL	NULL	NULL	NULL	presence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dependence on Ca2 + and tropomyosin of the actin-activated ATPase activity of phosphorylated gizzard myosin in the presence of low concentrations of Mg2 + .
	manualset3
261221	6	426167	7	NULL	NULL	NULL	NULL	low concentrations	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dependence on Ca2 + and tropomyosin of the actin-activated ATPase activity of phosphorylated gizzard myosin in the presence of low concentrations of Mg2 + .
	manualset3
261223	7	426167	7	NULL	NULL	NULL	NULL	Mg2 +	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dependence on Ca2 + and tropomyosin of the actin-activated ATPase activity of phosphorylated gizzard myosin in the presence of low concentrations of Mg2 + .
	manualset3
261484	1	426168	7	NULL	NULL	NULL	NULL	 characteristics	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the characteristics of each paired-pigment species , naturally occurring changes in visual pigment ratios are related to migrations in anadromous and catadromous teleosts and anadromous cyclostomes and to seasonal variation in several teleosts .
	manualset3
261495	2	426168	7	NULL	NULL	NULL	NULL	paired-pigment species	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the characteristics of each paired-pigment species , naturally occurring changes in visual pigment ratios are related to migrations in anadromous and catadromous teleosts and anadromous cyclostomes and to seasonal variation in several teleosts .
	manualset3
261500	3	426168	7	NULL	NULL	NULL	NULL	 naturally occurring  changes 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the characteristics of each paired-pigment species , naturally occurring changes in visual pigment ratios are related to migrations in anadromous and catadromous teleosts and anadromous cyclostomes and to seasonal variation in several teleosts .
	manualset3
261501	4	426168	7	NULL	NULL	NULL	NULL	visual pigment ratios	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the characteristics of each paired-pigment species , naturally occurring changes in visual pigment ratios are related to migrations in anadromous and catadromous teleosts and anadromous cyclostomes and to seasonal variation in several teleosts .
	manualset3
261502	5	426168	7	NULL	NULL	NULL	NULL	migrations 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the characteristics of each paired-pigment species , naturally occurring changes in visual pigment ratios are related to migrations in anadromous and catadromous teleosts and anadromous cyclostomes and to seasonal variation in several teleosts .
	manualset3
261529	6	426168	7	NULL	NULL	NULL	NULL	anadromous teleosts	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the characteristics of each paired-pigment species , naturally occurring changes in visual pigment ratios are related to migrations in anadromous and catadromous teleosts and anadromous cyclostomes and to seasonal variation in several teleosts .
	manualset3
261530	7	426168	7	NULL	NULL	NULL	NULL	catadromous teleosts	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the characteristics of each paired-pigment species , naturally occurring changes in visual pigment ratios are related to migrations in anadromous and catadromous teleosts and anadromous cyclostomes and to seasonal variation in several teleosts .
	manualset3
261532	8	426168	7	NULL	NULL	NULL	NULL	anadromous cyclostomes	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the characteristics of each paired-pigment species , naturally occurring changes in visual pigment ratios are related to migrations in anadromous and catadromous teleosts and anadromous cyclostomes and to seasonal variation in several teleosts .
	manualset3
261533	9	426168	7	NULL	NULL	NULL	NULL	seasonal variation 	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the characteristics of each paired-pigment species , naturally occurring changes in visual pigment ratios are related to migrations in anadromous and catadromous teleosts and anadromous cyclostomes and to seasonal variation in several teleosts .
	manualset3
261534	10	426168	7	NULL	NULL	NULL	NULL	several teleosts	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the characteristics of each paired-pigment species , naturally occurring changes in visual pigment ratios are related to migrations in anadromous and catadromous teleosts and anadromous cyclostomes and to seasonal variation in several teleosts .
	manualset3
261847	1	426170	7	NULL	NULL	NULL	NULL	nature	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the nature of the guest , shifts in the effective basicities of the encapsulated amines of up to 4.5 pK ( a ) units are observed , signifying a substantial stabilization of the protonated form of the guest molecule and effectively making phosphines and amines strong bases .
	manualset3
261854	2	426170	7	NULL	NULL	NULL	NULL	 guest	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the nature of the guest , shifts in the effective basicities of the encapsulated amines of up to 4.5 pK ( a ) units are observed , signifying a substantial stabilization of the protonated form of the guest molecule and effectively making phosphines and amines strong bases .
	manualset3
261861	3	426170	7	NULL	NULL	NULL	NULL	shifts	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the nature of the guest , shifts in the effective basicities of the encapsulated amines of up to 4.5 pK ( a ) units are observed , signifying a substantial stabilization of the protonated form of the guest molecule and effectively making phosphines and amines strong bases .
	manualset3
261863	4	426170	7	NULL	NULL	NULL	NULL	effective basicities	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the nature of the guest , shifts in the effective basicities of the encapsulated amines of up to 4.5 pK ( a ) units are observed , signifying a substantial stabilization of the protonated form of the guest molecule and effectively making phosphines and amines strong bases .
	manualset3
261865	5	426170	7	NULL	NULL	NULL	NULL	encapsulated amines	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the nature of the guest , shifts in the effective basicities of the encapsulated amines of up to 4.5 pK ( a ) units are observed , signifying a substantial stabilization of the protonated form of the guest molecule and effectively making phosphines and amines strong bases .
	manualset3
261868	6	426170	7	NULL	NULL	NULL	NULL	 4.5 pK ( a ) units	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the nature of the guest , shifts in the effective basicities of the encapsulated amines of up to 4.5 pK ( a ) units are observed , signifying a substantial stabilization of the protonated form of the guest molecule and effectively making phosphines and amines strong bases .
	manualset3
261870	7	426170	7	NULL	NULL	NULL	NULL	substantial stabilization	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the nature of the guest , shifts in the effective basicities of the encapsulated amines of up to 4.5 pK ( a ) units are observed , signifying a substantial stabilization of the protonated form of the guest molecule and effectively making phosphines and amines strong bases .
	manualset3
261872	8	426170	7	NULL	NULL	NULL	NULL	protonated form	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the nature of the guest , shifts in the effective basicities of the encapsulated amines of up to 4.5 pK ( a ) units are observed , signifying a substantial stabilization of the protonated form of the guest molecule and effectively making phosphines and amines strong bases .
	manualset3
261875	9	426170	7	NULL	NULL	NULL	NULL	guest molecule 	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the nature of the guest , shifts in the effective basicities of the encapsulated amines of up to 4.5 pK ( a ) units are observed , signifying a substantial stabilization of the protonated form of the guest molecule and effectively making phosphines and amines strong bases .
	manualset3
261877	10	426170	7	NULL	NULL	NULL	NULL	phosphines	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the nature of the guest , shifts in the effective basicities of the encapsulated amines of up to 4.5 pK ( a ) units are observed , signifying a substantial stabilization of the protonated form of the guest molecule and effectively making phosphines and amines strong bases .
	manualset3
261880	11	426170	7	NULL	NULL	NULL	NULL	amines	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the nature of the guest , shifts in the effective basicities of the encapsulated amines of up to 4.5 pK ( a ) units are observed , signifying a substantial stabilization of the protonated form of the guest molecule and effectively making phosphines and amines strong bases .
	manualset3
261883	12	426170	7	NULL	NULL	NULL	NULL	strong bases	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the nature of the guest , shifts in the effective basicities of the encapsulated amines of up to 4.5 pK ( a ) units are observed , signifying a substantial stabilization of the protonated form of the guest molecule and effectively making phosphines and amines strong bases .
	manualset3
261888	1	426171	7	NULL	NULL	NULL	NULL	orientation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the orientation of the G segment , two types of phage particles , G ( + ) and G ( - ) , are produced which recognize different cell surface receptors .
	manualset3
261889	2	426171	7	NULL	NULL	NULL	NULL	G segment 	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the orientation of the G segment , two types of phage particles , G ( + ) and G ( - ) , are produced which recognize different cell surface receptors .
	manualset3
261890	3	426171	7	NULL	NULL	NULL	NULL	 two types	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the orientation of the G segment , two types of phage particles , G ( + ) and G ( - ) , are produced which recognize different cell surface receptors .
	manualset3
261891	4	426171	7	NULL	NULL	NULL	NULL	phage particles	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the orientation of the G segment , two types of phage particles , G ( + ) and G ( - ) , are produced which recognize different cell surface receptors .
	manualset3
261892	5	426171	7	NULL	NULL	NULL	NULL	G ( + ) 	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the orientation of the G segment , two types of phage particles , G ( + ) and G ( - ) , are produced which recognize different cell surface receptors .
	manualset3
261893	6	426171	7	NULL	NULL	NULL	NULL	G ( - ) 	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the orientation of the G segment , two types of phage particles , G ( + ) and G ( - ) , are produced which recognize different cell surface receptors .
	manualset3
261894	7	426171	7	NULL	NULL	NULL	NULL	cell surface receptors	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the orientation of the G segment , two types of phage particles , G ( + ) and G ( - ) , are produced which recognize different cell surface receptors .
	manualset3
261895	1	426172	7	NULL	NULL	NULL	NULL	Nervous system	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Nervous system of the kidney ) .
	manualset3
261896	2	426172	7	NULL	NULL	NULL	NULL	kidney	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Nervous system of the kidney ) .
	manualset3
261897	1	426173	7	NULL	NULL	NULL	NULL	 stimuli	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the stimuli they encounter , B lymphocytes engage in signaling events that lead to immunity or tolerance .
	manualset3
261898	2	426173	7	NULL	NULL	NULL	NULL	B lymphocytes	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the stimuli they encounter , B lymphocytes engage in signaling events that lead to immunity or tolerance .
	manualset3
261899	3	426173	7	NULL	NULL	NULL	NULL	signaling events	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the stimuli they encounter , B lymphocytes engage in signaling events that lead to immunity or tolerance .
	manualset3
261900	4	426173	7	NULL	NULL	NULL	NULL	immunity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the stimuli they encounter , B lymphocytes engage in signaling events that lead to immunity or tolerance .
	manualset3
261901	5	426173	7	NULL	NULL	NULL	NULL	 tolerance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the stimuli they encounter , B lymphocytes engage in signaling events that lead to immunity or tolerance .
	manualset3
261902	1	426174	7	NULL	NULL	NULL	NULL	 stimulus	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the stimulus , the phenotype of macrophage activation is broadly classified into M1 ( NOS2 ( + ) ) and M2 ( arginase-1 ( + ) ) .
	manualset3
261903	2	426174	7	NULL	NULL	NULL	NULL	 phenotype	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the stimulus , the phenotype of macrophage activation is broadly classified into M1 ( NOS2 ( + ) ) and M2 ( arginase-1 ( + ) ) .
	manualset3
261904	3	426174	7	NULL	NULL	NULL	NULL	macrophage activation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the stimulus , the phenotype of macrophage activation is broadly classified into M1 ( NOS2 ( + ) ) and M2 ( arginase-1 ( + ) ) .
	manualset3
261905	4	426174	7	NULL	NULL	NULL	NULL	M1 ( NOS2 ( + ) ) 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the stimulus , the phenotype of macrophage activation is broadly classified into M1 ( NOS2 ( + ) ) and M2 ( arginase-1 ( + ) ) .
	manualset3
261906	5	426174	7	NULL	NULL	NULL	NULL	M2 ( arginase-1 ( + ) )	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depending on the stimulus , the phenotype of macrophage activation is broadly classified into M1 ( NOS2 ( + ) ) and M2 ( arginase-1 ( + ) ) .
	manualset3
261907	1	426175	7	NULL	NULL	NULL	NULL	Depleted iron stores	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depleted iron stores without anemia early in pregnancy carries increased risk of lower birthweight even when supplemented daily with moderate iron .
	manualset3
261908	2	426175	7	NULL	NULL	NULL	NULL	anemia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depleted iron stores without anemia early in pregnancy carries increased risk of lower birthweight even when supplemented daily with moderate iron .
	manualset3
261909	3	426175	7	NULL	NULL	NULL	NULL	pregnancy	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depleted iron stores without anemia early in pregnancy carries increased risk of lower birthweight even when supplemented daily with moderate iron .
	manualset3
261910	4	426175	7	NULL	NULL	NULL	NULL	 increased risk	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depleted iron stores without anemia early in pregnancy carries increased risk of lower birthweight even when supplemented daily with moderate iron .
	manualset3
261911	5	426175	7	NULL	NULL	NULL	NULL	lower birthweight 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depleted iron stores without anemia early in pregnancy carries increased risk of lower birthweight even when supplemented daily with moderate iron .
	manualset3
261912	6	426175	7	NULL	NULL	NULL	NULL	moderate iron	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depleted iron stores without anemia early in pregnancy carries increased risk of lower birthweight even when supplemented daily with moderate iron .
	manualset3
261913	7	426175	7	NULL	NULL	NULL	NULL	early	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depleted iron stores without anemia early in pregnancy carries increased risk of lower birthweight even when supplemented daily with moderate iron .
	manualset3
261914	1	426176	7	NULL	NULL	NULL	NULL	Depletion	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depletion caused a more dramatic increase in PGE2 production than did activation , suggesting that Mac-1 + M luminal diameter had a dampening effect on PGE2 production .
	manualset3
261915	2	426176	7	NULL	NULL	NULL	NULL	increase	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depletion caused a more dramatic increase in PGE2 production than did activation , suggesting that Mac-1 + M luminal diameter had a dampening effect on PGE2 production .
	manualset3
261916	3	426176	7	NULL	NULL	NULL	NULL	PGE2 production 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depletion caused a more dramatic increase in PGE2 production than did activation , suggesting that Mac-1 + M luminal diameter had a dampening effect on PGE2 production .
	manualset3
261917	4	426176	7	NULL	NULL	NULL	NULL	activation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depletion caused a more dramatic increase in PGE2 production than did activation , suggesting that Mac-1 + M luminal diameter had a dampening effect on PGE2 production .
	manualset3
261918	5	426176	7	NULL	NULL	NULL	NULL	Mac-1 + M luminal diameter	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depletion caused a more dramatic increase in PGE2 production than did activation , suggesting that Mac-1 + M luminal diameter had a dampening effect on PGE2 production .
	manualset3
261919	6	426176	7	NULL	NULL	NULL	NULL	dampening effect 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depletion caused a more dramatic increase in PGE2 production than did activation , suggesting that Mac-1 + M luminal diameter had a dampening effect on PGE2 production .
	manualset3
261920	7	426176	7	NULL	NULL	NULL	NULL	PGE2 production	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depletion caused a more dramatic increase in PGE2 production than did activation , suggesting that Mac-1 + M luminal diameter had a dampening effect on PGE2 production .
	manualset3
261921	1	426177	7	NULL	NULL	NULL	NULL	Depletion	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depletion of FADD , caspase-8 , BID , or BAX and BAK but not RIP3 attenuated TWEAK-induced cell death .
	manualset3
261922	2	426177	7	NULL	NULL	NULL	NULL	 FADD	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depletion of FADD , caspase-8 , BID , or BAX and BAK but not RIP3 attenuated TWEAK-induced cell death .
	manualset3
261923	3	426177	7	NULL	NULL	NULL	NULL	 caspase-8	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depletion of FADD , caspase-8 , BID , or BAX and BAK but not RIP3 attenuated TWEAK-induced cell death .
	manualset3
261924	4	426177	7	NULL	NULL	NULL	NULL	BID	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depletion of FADD , caspase-8 , BID , or BAX and BAK but not RIP3 attenuated TWEAK-induced cell death .
	manualset3
261925	5	426177	7	NULL	NULL	NULL	NULL	BAX	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depletion of FADD , caspase-8 , BID , or BAX and BAK but not RIP3 attenuated TWEAK-induced cell death .
	manualset3
261926	6	426177	7	NULL	NULL	NULL	NULL	BAK	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depletion of FADD , caspase-8 , BID , or BAX and BAK but not RIP3 attenuated TWEAK-induced cell death .
	manualset3
261927	7	426177	7	NULL	NULL	NULL	NULL	RIP3	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depletion of FADD , caspase-8 , BID , or BAX and BAK but not RIP3 attenuated TWEAK-induced cell death .
	manualset3
261928	8	426177	7	NULL	NULL	NULL	NULL	TWEAK-induced cell death	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Depletion of FADD , caspase-8 , BID , or BAX and BAK but not RIP3 attenuated TWEAK-induced cell death .
	manualset3
261929	1	426178	7	NULL	NULL	NULL	NULL	Deposition	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deposition of cationic polymer micelles on planar SiO2 surfaces .
	manualset3
261930	2	426178	7	NULL	NULL	NULL	NULL	cationic polymer micelles	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deposition of cationic polymer micelles on planar SiO2 surfaces .
	manualset3
261931	3	426178	7	NULL	NULL	NULL	NULL	planar SiO2 surfaces	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deposition of cationic polymer micelles on planar SiO2 surfaces .
	manualset3
261932	1	426179	7	NULL	NULL	NULL	NULL	Deprivation indices	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deprivation indices , population health and geography : an evaluation of the spatial effectiveness of indices at multiple scales .
	manualset3
261933	2	426179	7	NULL	NULL	NULL	NULL	population health 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deprivation indices , population health and geography : an evaluation of the spatial effectiveness of indices at multiple scales .
	manualset3
261934	3	426179	7	NULL	NULL	NULL	NULL	 geography	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deprivation indices , population health and geography : an evaluation of the spatial effectiveness of indices at multiple scales .
	manualset3
261935	4	426179	7	NULL	NULL	NULL	NULL	evaluation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deprivation indices , population health and geography : an evaluation of the spatial effectiveness of indices at multiple scales .
	manualset3
261936	5	426179	7	NULL	NULL	NULL	NULL	spatial effectiveness	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deprivation indices , population health and geography : an evaluation of the spatial effectiveness of indices at multiple scales .
	manualset3
261937	6	426179	7	NULL	NULL	NULL	NULL	indices	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deprivation indices , population health and geography : an evaluation of the spatial effectiveness of indices at multiple scales .
	manualset3
261938	7	426179	7	NULL	NULL	NULL	NULL	multiple scales	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deprivation indices , population health and geography : an evaluation of the spatial effectiveness of indices at multiple scales .
	manualset3
261939	1	426180	7	NULL	NULL	NULL	NULL	Deprived eye responses	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deprived eye responses decreased after MD , whereas nondeprived eye responses increased .
	manualset3
261940	2	426180	7	NULL	NULL	NULL	NULL	MD	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deprived eye responses decreased after MD , whereas nondeprived eye responses increased .
	manualset3
261941	3	426180	7	NULL	NULL	NULL	NULL	nondeprived eye responses	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Deprived eye responses decreased after MD , whereas nondeprived eye responses increased .
	manualset3
261942	1	426181	7	NULL	NULL	NULL	NULL	Neuromuscular transmission 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Neuromuscular transmission after gangliectomy in crayfish ) .
	manualset3
261943	2	426181	7	NULL	NULL	NULL	NULL	gangliectomy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Neuromuscular transmission after gangliectomy in crayfish ) .
	manualset3
261944	3	426181	7	NULL	NULL	NULL	NULL	crayfish	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Neuromuscular transmission after gangliectomy in crayfish ) .
	manualset3
261945	1	426182	7	NULL	NULL	NULL	NULL	Derangements	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Derangements of mucinase activity lead to downstream barrier defects and mucosal disease .
	manualset3
261946	2	426182	7	NULL	NULL	NULL	NULL	 mucinase activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Derangements of mucinase activity lead to downstream barrier defects and mucosal disease .
	manualset3
261947	3	426182	7	NULL	NULL	NULL	NULL	barrier defects	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Derangements of mucinase activity lead to downstream barrier defects and mucosal disease .
	manualset3
261948	4	426182	7	NULL	NULL	NULL	NULL	 mucosal disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Derangements of mucinase activity lead to downstream barrier defects and mucosal disease .
	manualset3
261949	1	426183	7	NULL	NULL	NULL	NULL	Dermal papillae	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dermal papillae from both clinically normal and lesional alopecia areata follicles were less well organized and the dermal papilla cells exhibited signs of cell injury and contained abnormal amounts of pigment ; an increased concentration of fibrous material in the extracellular matrix and thickening of the dermal papilla-epithelial junction were also seen .
	manualset3
261950	2	426183	7	NULL	NULL	NULL	NULL	clinically normal alopecia areata follicles	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dermal papillae from both clinically normal and lesional alopecia areata follicles were less well organized and the dermal papilla cells exhibited signs of cell injury and contained abnormal amounts of pigment ; an increased concentration of fibrous material in the extracellular matrix and thickening of the dermal papilla-epithelial junction were also seen .
	manualset3
261951	3	426183	7	NULL	NULL	NULL	NULL	lesional alopecia areata follicles	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dermal papillae from both clinically normal and lesional alopecia areata follicles were less well organized and the dermal papilla cells exhibited signs of cell injury and contained abnormal amounts of pigment ; an increased concentration of fibrous material in the extracellular matrix and thickening of the dermal papilla-epithelial junction were also seen .
	manualset3
261952	4	426183	7	NULL	NULL	NULL	NULL	dermal papilla cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dermal papillae from both clinically normal and lesional alopecia areata follicles were less well organized and the dermal papilla cells exhibited signs of cell injury and contained abnormal amounts of pigment ; an increased concentration of fibrous material in the extracellular matrix and thickening of the dermal papilla-epithelial junction were also seen .
	manualset3
261953	5	426183	7	NULL	NULL	NULL	NULL	signs	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dermal papillae from both clinically normal and lesional alopecia areata follicles were less well organized and the dermal papilla cells exhibited signs of cell injury and contained abnormal amounts of pigment ; an increased concentration of fibrous material in the extracellular matrix and thickening of the dermal papilla-epithelial junction were also seen .
	manualset3
261954	6	426183	7	NULL	NULL	NULL	NULL	cell injury	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dermal papillae from both clinically normal and lesional alopecia areata follicles were less well organized and the dermal papilla cells exhibited signs of cell injury and contained abnormal amounts of pigment ; an increased concentration of fibrous material in the extracellular matrix and thickening of the dermal papilla-epithelial junction were also seen .
	manualset3
261955	7	426183	7	NULL	NULL	NULL	NULL	abnormal amounts	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dermal papillae from both clinically normal and lesional alopecia areata follicles were less well organized and the dermal papilla cells exhibited signs of cell injury and contained abnormal amounts of pigment ; an increased concentration of fibrous material in the extracellular matrix and thickening of the dermal papilla-epithelial junction were also seen .
	manualset3
261956	8	426183	7	NULL	NULL	NULL	NULL	pigment 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dermal papillae from both clinically normal and lesional alopecia areata follicles were less well organized and the dermal papilla cells exhibited signs of cell injury and contained abnormal amounts of pigment ; an increased concentration of fibrous material in the extracellular matrix and thickening of the dermal papilla-epithelial junction were also seen .
	manualset3
261957	9	426183	7	NULL	NULL	NULL	NULL	 increased concentration	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dermal papillae from both clinically normal and lesional alopecia areata follicles were less well organized and the dermal papilla cells exhibited signs of cell injury and contained abnormal amounts of pigment ; an increased concentration of fibrous material in the extracellular matrix and thickening of the dermal papilla-epithelial junction were also seen .
	manualset3
261958	10	426183	7	NULL	NULL	NULL	NULL	fibrous material	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dermal papillae from both clinically normal and lesional alopecia areata follicles were less well organized and the dermal papilla cells exhibited signs of cell injury and contained abnormal amounts of pigment ; an increased concentration of fibrous material in the extracellular matrix and thickening of the dermal papilla-epithelial junction were also seen .
	manualset3
261959	11	426183	7	NULL	NULL	NULL	NULL	extracellular matrix	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dermal papillae from both clinically normal and lesional alopecia areata follicles were less well organized and the dermal papilla cells exhibited signs of cell injury and contained abnormal amounts of pigment ; an increased concentration of fibrous material in the extracellular matrix and thickening of the dermal papilla-epithelial junction were also seen .
	manualset3
261960	12	426183	7	NULL	NULL	NULL	NULL	thickening 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dermal papillae from both clinically normal and lesional alopecia areata follicles were less well organized and the dermal papilla cells exhibited signs of cell injury and contained abnormal amounts of pigment ; an increased concentration of fibrous material in the extracellular matrix and thickening of the dermal papilla-epithelial junction were also seen .
	manualset3
261961	13	426183	7	NULL	NULL	NULL	NULL	 dermal papilla-epithelial junction	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dermal papillae from both clinically normal and lesional alopecia areata follicles were less well organized and the dermal papilla cells exhibited signs of cell injury and contained abnormal amounts of pigment ; an increased concentration of fibrous material in the extracellular matrix and thickening of the dermal papilla-epithelial junction were also seen .
	manualset3
261962	1	426184	7	NULL	NULL	NULL	NULL	Desacetylmethylcolchicine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Desacetylmethylcolchicine in the treatment of leukemia .
	manualset3
261963	2	426184	7	NULL	NULL	NULL	NULL	treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Desacetylmethylcolchicine in the treatment of leukemia .
	manualset3
261964	3	426184	7	NULL	NULL	NULL	NULL	leukemia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Desacetylmethylcolchicine in the treatment of leukemia .
	manualset3
261965	1	426185	7	NULL	NULL	NULL	NULL	long-spinal excitation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Descending long-spinal excitation of lumbar alpha and gamma motoneurons evoked by stretch of dorsal neck muscles .
	manualset3
261966	2	426185	7	NULL	NULL	NULL	NULL	 lumbar alpha motoneurons	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Descending long-spinal excitation of lumbar alpha and gamma motoneurons evoked by stretch of dorsal neck muscles .
	manualset3
261967	3	426185	7	NULL	NULL	NULL	NULL	gamma motoneurons 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Descending long-spinal excitation of lumbar alpha and gamma motoneurons evoked by stretch of dorsal neck muscles .
	manualset3
261968	4	426185	7	NULL	NULL	NULL	NULL	stretch	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Descending long-spinal excitation of lumbar alpha and gamma motoneurons evoked by stretch of dorsal neck muscles .
	manualset3
261969	5	426185	7	NULL	NULL	NULL	NULL	dorsal neck muscles	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Descending long-spinal excitation of lumbar alpha and gamma motoneurons evoked by stretch of dorsal neck muscles .
	manualset3
261970	1	426186	7	NULL	NULL	NULL	NULL	 brief rationale	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Described here is a brief rationale for applying a public health approach to child maltreatment and a discussion of the priority-setting process , priorities in each of four areas of the public health model , and some of CDC 's current child maltreatment prevention activities .
	manualset3
261971	2	426186	7	NULL	NULL	NULL	NULL	 public health approach	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Described here is a brief rationale for applying a public health approach to child maltreatment and a discussion of the priority-setting process , priorities in each of four areas of the public health model , and some of CDC 's current child maltreatment prevention activities .
	manualset3
261972	3	426186	7	NULL	NULL	NULL	NULL	child maltreatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Described here is a brief rationale for applying a public health approach to child maltreatment and a discussion of the priority-setting process , priorities in each of four areas of the public health model , and some of CDC 's current child maltreatment prevention activities .
	manualset3
261973	4	426186	7	NULL	NULL	NULL	NULL	discussion	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Described here is a brief rationale for applying a public health approach to child maltreatment and a discussion of the priority-setting process , priorities in each of four areas of the public health model , and some of CDC 's current child maltreatment prevention activities .
	manualset3
261974	5	426186	7	NULL	NULL	NULL	NULL	 priority-setting process 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Described here is a brief rationale for applying a public health approach to child maltreatment and a discussion of the priority-setting process , priorities in each of four areas of the public health model , and some of CDC 's current child maltreatment prevention activities .
	manualset3
261975	6	426186	7	NULL	NULL	NULL	NULL	 four areas	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Described here is a brief rationale for applying a public health approach to child maltreatment and a discussion of the priority-setting process , priorities in each of four areas of the public health model , and some of CDC 's current child maltreatment prevention activities .
	manualset3
261976	7	426186	7	NULL	NULL	NULL	NULL	public health model	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Described here is a brief rationale for applying a public health approach to child maltreatment and a discussion of the priority-setting process , priorities in each of four areas of the public health model , and some of CDC 's current child maltreatment prevention activities .
	manualset3
261977	8	426186	7	NULL	NULL	NULL	NULL	 CDC 's current child maltreatment prevention activities	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Described here is a brief rationale for applying a public health approach to child maltreatment and a discussion of the priority-setting process , priorities in each of four areas of the public health model , and some of CDC 's current child maltreatment prevention activities .
	manualset3
261978	1	426187	7	NULL	NULL	NULL	NULL	Descriptions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Descriptions of MSG-induced asthma , urticaria , angio-oedema , and rhinitis have prompted some to suggest that MSG should be an aetiologic consideration in patients presenting with these conditions .
	manualset3
261979	2	426187	7	NULL	NULL	NULL	NULL	MSG-induced asthma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Descriptions of MSG-induced asthma , urticaria , angio-oedema , and rhinitis have prompted some to suggest that MSG should be an aetiologic consideration in patients presenting with these conditions .
	manualset3
261980	3	426187	7	NULL	NULL	NULL	NULL	 urticaria	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Descriptions of MSG-induced asthma , urticaria , angio-oedema , and rhinitis have prompted some to suggest that MSG should be an aetiologic consideration in patients presenting with these conditions .
	manualset3
261981	4	426187	7	NULL	NULL	NULL	NULL	angio-oedema	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Descriptions of MSG-induced asthma , urticaria , angio-oedema , and rhinitis have prompted some to suggest that MSG should be an aetiologic consideration in patients presenting with these conditions .
	manualset3
261982	5	426187	7	NULL	NULL	NULL	NULL	rhinitis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Descriptions of MSG-induced asthma , urticaria , angio-oedema , and rhinitis have prompted some to suggest that MSG should be an aetiologic consideration in patients presenting with these conditions .
	manualset3
261983	6	426187	7	NULL	NULL	NULL	NULL	MSG	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Descriptions of MSG-induced asthma , urticaria , angio-oedema , and rhinitis have prompted some to suggest that MSG should be an aetiologic consideration in patients presenting with these conditions .
	manualset3
261984	7	426187	7	NULL	NULL	NULL	NULL	aetiologic consideration	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Descriptions of MSG-induced asthma , urticaria , angio-oedema , and rhinitis have prompted some to suggest that MSG should be an aetiologic consideration in patients presenting with these conditions .
	manualset3
261985	8	426187	7	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Descriptions of MSG-induced asthma , urticaria , angio-oedema , and rhinitis have prompted some to suggest that MSG should be an aetiologic consideration in patients presenting with these conditions .
	manualset3
261986	9	426187	7	NULL	NULL	NULL	NULL	conditions	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Descriptions of MSG-induced asthma , urticaria , angio-oedema , and rhinitis have prompted some to suggest that MSG should be an aetiologic consideration in patients presenting with these conditions .
	manualset3
261987	1	426188	7	NULL	NULL	NULL	NULL	Neuropsychological study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Neuropsychological study of the senile brain during and after single and combined treatment with deanol and citicoline ) .
	manualset3
261988	2	426188	7	NULL	NULL	NULL	NULL	senile brain	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Neuropsychological study of the senile brain during and after single and combined treatment with deanol and citicoline ) .
	manualset3
261989	3	426188	7	NULL	NULL	NULL	NULL	single treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Neuropsychological study of the senile brain during and after single and combined treatment with deanol and citicoline ) .
	manualset3
261990	4	426188	7	NULL	NULL	NULL	NULL	combined treatment 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Neuropsychological study of the senile brain during and after single and combined treatment with deanol and citicoline ) .
	manualset3
261991	5	426188	7	NULL	NULL	NULL	NULL	deanol 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Neuropsychological study of the senile brain during and after single and combined treatment with deanol and citicoline ) .
	manualset3
261992	6	426188	7	NULL	NULL	NULL	NULL	citicoline	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Neuropsychological study of the senile brain during and after single and combined treatment with deanol and citicoline ) .
	manualset3
261993	1	426189	7	NULL	NULL	NULL	NULL	Descriptive norms 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Descriptive norms , personal drinking values , and alcohol expectancies were robust mediators of broad social motives for both alcohol use and problems .
	manualset3
261994	2	426189	7	NULL	NULL	NULL	NULL	 personal drinking values 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Descriptive norms , personal drinking values , and alcohol expectancies were robust mediators of broad social motives for both alcohol use and problems .
	manualset3
261995	3	426189	7	NULL	NULL	NULL	NULL	alcohol expectancies	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Descriptive norms , personal drinking values , and alcohol expectancies were robust mediators of broad social motives for both alcohol use and problems .
	manualset3
261996	4	426189	7	NULL	NULL	NULL	NULL	mediators 	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Descriptive norms , personal drinking values , and alcohol expectancies were robust mediators of broad social motives for both alcohol use and problems .
	manualset3
261997	5	426189	7	NULL	NULL	NULL	NULL	broad social motives	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Descriptive norms , personal drinking values , and alcohol expectancies were robust mediators of broad social motives for both alcohol use and problems .
	manualset3
261998	6	426189	7	NULL	NULL	NULL	NULL	alcohol use	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Descriptive norms , personal drinking values , and alcohol expectancies were robust mediators of broad social motives for both alcohol use and problems .
	manualset3
261999	7	426189	7	NULL	NULL	NULL	NULL	problems	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Descriptive norms , personal drinking values , and alcohol expectancies were robust mediators of broad social motives for both alcohol use and problems .
	manualset3
262000	1	426190	7	NULL	NULL	NULL	NULL	Design 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Design , synthesis , and anti-influenza viral activities of 1 , 3-diarylprop-2-en-1-ones : A novel class of neuraminidase inhibitors .
	manualset3
262001	2	426190	7	NULL	NULL	NULL	NULL	synthesis	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Design , synthesis , and anti-influenza viral activities of 1 , 3-diarylprop-2-en-1-ones : A novel class of neuraminidase inhibitors .
	manualset3
262002	3	426190	7	NULL	NULL	NULL	NULL	anti-influenza viral activities 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Design , synthesis , and anti-influenza viral activities of 1 , 3-diarylprop-2-en-1-ones : A novel class of neuraminidase inhibitors .
	manualset3
262003	4	426190	7	NULL	NULL	NULL	NULL	1 , 3-diarylprop-2-en-1-ones	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Design , synthesis , and anti-influenza viral activities of 1 , 3-diarylprop-2-en-1-ones : A novel class of neuraminidase inhibitors .
	manualset3
262004	5	426190	7	NULL	NULL	NULL	NULL	novel class	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Design , synthesis , and anti-influenza viral activities of 1 , 3-diarylprop-2-en-1-ones : A novel class of neuraminidase inhibitors .
	manualset3
262005	6	426190	7	NULL	NULL	NULL	NULL	neuraminidase inhibitors	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Design , synthesis , and anti-influenza viral activities of 1 , 3-diarylprop-2-en-1-ones : A novel class of neuraminidase inhibitors .
	manualset3
262006	1	426191	7	NULL	NULL	NULL	NULL	Design 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Design and characterization of dual-curvature 1.5-dimensional high-intensity focused ultrasound phased-array transducer .
	manualset3
262007	2	426191	7	NULL	NULL	NULL	NULL	characterization 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Design and characterization of dual-curvature 1.5-dimensional high-intensity focused ultrasound phased-array transducer .
	manualset3
262008	3	426191	7	NULL	NULL	NULL	NULL	dual-curvature 1.5-dimensional high-intensity focused ultrasound phased-array transducer	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Design and characterization of dual-curvature 1.5-dimensional high-intensity focused ultrasound phased-array transducer .
	manualset3
262009	1	426192	7	NULL	NULL	NULL	NULL	Design	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Design and logistics of lifetime carcinogenesis bioassay using Syrian hamsters .
	manualset3
262010	2	426192	7	NULL	NULL	NULL	NULL	 logistics	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Design and logistics of lifetime carcinogenesis bioassay using Syrian hamsters .
	manualset3
262011	3	426192	7	NULL	NULL	NULL	NULL	 lifetime carcinogenesis bioassay	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Design and logistics of lifetime carcinogenesis bioassay using Syrian hamsters .
	manualset3
262012	4	426192	7	NULL	NULL	NULL	NULL	Syrian hamsters	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Design and logistics of lifetime carcinogenesis bioassay using Syrian hamsters .
	manualset3
262013	1	426193	7	NULL	NULL	NULL	NULL	Designed multiple ligands 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Designed multiple ligands : an emerging anti-HIV drug discovery paradigm .
	manualset3
262014	2	426193	7	NULL	NULL	NULL	NULL	anti-HIV drug discovery paradigm	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Designed multiple ligands : an emerging anti-HIV drug discovery paradigm .
	manualset3
262015	1	426194	7	NULL	NULL	NULL	NULL	protein mimics 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Designed protein mimics of the Ebola virus glycoprotein GP2 - helical bundle : stability and pH effects .
	manualset3
262016	2	426194	7	NULL	NULL	NULL	NULL	Ebola virus glycoprotein GP2 - helical bundle	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Designed protein mimics of the Ebola virus glycoprotein GP2 - helical bundle : stability and pH effects .
	manualset3
262017	3	426194	7	NULL	NULL	NULL	NULL	stability	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Designed protein mimics of the Ebola virus glycoprotein GP2 - helical bundle : stability and pH effects .
	manualset3
262018	4	426194	7	NULL	NULL	NULL	NULL	 pH effects	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Designed protein mimics of the Ebola virus glycoprotein GP2 - helical bundle : stability and pH effects .
	manualset3
262019	1	426195	7	NULL	NULL	NULL	NULL	 New antibiotics	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( New antibiotics in the service of the surgeon ) .
	manualset3
262020	2	426195	7	NULL	NULL	NULL	NULL	 service	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( New antibiotics in the service of the surgeon ) .
	manualset3
262021	3	426195	7	NULL	NULL	NULL	NULL	 surgeon	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( New antibiotics in the service of the surgeon ) .
	manualset3
262022	1	426196	7	NULL	NULL	NULL	NULL	new UK-WHO growth charts	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Designing new UK-WHO growth charts : implications for health staff use and understanding of charts and growth monitoring .
	manualset3
262023	2	426196	7	NULL	NULL	NULL	NULL	 implications	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Designing new UK-WHO growth charts : implications for health staff use and understanding of charts and growth monitoring .
	manualset3
262024	3	426196	7	NULL	NULL	NULL	NULL	health staff use	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Designing new UK-WHO growth charts : implications for health staff use and understanding of charts and growth monitoring .
	manualset3
262025	4	426196	7	NULL	NULL	NULL	NULL	understanding	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Designing new UK-WHO growth charts : implications for health staff use and understanding of charts and growth monitoring .
	manualset3
262026	5	426196	7	NULL	NULL	NULL	NULL	charts 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Designing new UK-WHO growth charts : implications for health staff use and understanding of charts and growth monitoring .
	manualset3
262027	6	426196	7	NULL	NULL	NULL	NULL	growth monitoring 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Designing new UK-WHO growth charts : implications for health staff use and understanding of charts and growth monitoring .
	manualset3
262028	1	426197	7	NULL	NULL	NULL	NULL	new devices	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Designing new devices for measuring blood pressure .
	manualset3
262029	2	426197	7	NULL	NULL	NULL	NULL	blood pressure 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Designing new devices for measuring blood pressure .
	manualset3
262030	1	426198	7	NULL	NULL	NULL	NULL	decade	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite a decade of intensive investigation , the cellular mechanism ( s ) responsible for this paradoxical protection remain poorly understood .
	manualset3
262031	2	426198	7	NULL	NULL	NULL	NULL	intensive investigation	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite a decade of intensive investigation , the cellular mechanism ( s ) responsible for this paradoxical protection remain poorly understood .
	manualset3
262032	3	426198	7	NULL	NULL	NULL	NULL	cellular mechanism ( s )	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite a decade of intensive investigation , the cellular mechanism ( s ) responsible for this paradoxical protection remain poorly understood .
	manualset3
262033	4	426198	7	NULL	NULL	NULL	NULL	paradoxical protection	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite a decade of intensive investigation , the cellular mechanism ( s ) responsible for this paradoxical protection remain poorly understood .
	manualset3
262034	1	426199	7	NULL	NULL	NULL	NULL	similarity	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite a similarity in the initial intake , a significant ( p0 .05 ) increase in the final feed intake by the chicks with methionine addition was found in both rations .
	manualset3
262035	2	426199	7	NULL	NULL	NULL	NULL	initial intake	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite a similarity in the initial intake , a significant ( p0 .05 ) increase in the final feed intake by the chicks with methionine addition was found in both rations .
	manualset3
262036	3	426199	7	NULL	NULL	NULL	NULL	( p0 .05 )	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite a similarity in the initial intake , a significant ( p0 .05 ) increase in the final feed intake by the chicks with methionine addition was found in both rations .
	manualset3
262037	4	426199	7	NULL	NULL	NULL	NULL	 final feed intake	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite a similarity in the initial intake , a significant ( p0 .05 ) increase in the final feed intake by the chicks with methionine addition was found in both rations .
	manualset3
262038	5	426199	7	NULL	NULL	NULL	NULL	chicks	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite a similarity in the initial intake , a significant ( p0 .05 ) increase in the final feed intake by the chicks with methionine addition was found in both rations .
	manualset3
262039	6	426199	7	NULL	NULL	NULL	NULL	methionine addition	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite a similarity in the initial intake , a significant ( p0 .05 ) increase in the final feed intake by the chicks with methionine addition was found in both rations .
	manualset3
262040	7	426199	7	NULL	NULL	NULL	NULL	 rations	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite a similarity in the initial intake , a significant ( p0 .05 ) increase in the final feed intake by the chicks with methionine addition was found in both rations .
	manualset3
262041	8	426199	7	NULL	NULL	NULL	NULL	increase	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite a similarity in the initial intake , a significant ( p0 .05 ) increase in the final feed intake by the chicks with methionine addition was found in both rations .
	manualset3
262042	1	426200	7	NULL	NULL	NULL	NULL	 aggressive fixed-dose ( FD ) combination therapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite aggressive fixed-dose ( FD ) combination therapy with inhaled glucocorticosteroids ( ICS ) and long acting beta ( 2 ) - adrenoceptor agonists ( LABA ) , many patients with asthma remain suboptimally controlled , based on the need for rescue therapy and rates of severe exacerbations .
	manualset3
262043	2	426200	7	NULL	NULL	NULL	NULL	inhaled glucocorticosteroids ( ICS )	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite aggressive fixed-dose ( FD ) combination therapy with inhaled glucocorticosteroids ( ICS ) and long acting beta ( 2 ) - adrenoceptor agonists ( LABA ) , many patients with asthma remain suboptimally controlled , based on the need for rescue therapy and rates of severe exacerbations .
	manualset3
262044	3	426200	7	NULL	NULL	NULL	NULL	 long acting beta ( 2 ) - adrenoceptor agonists ( LABA )	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite aggressive fixed-dose ( FD ) combination therapy with inhaled glucocorticosteroids ( ICS ) and long acting beta ( 2 ) - adrenoceptor agonists ( LABA ) , many patients with asthma remain suboptimally controlled , based on the need for rescue therapy and rates of severe exacerbations .
	manualset3
262045	4	426200	7	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite aggressive fixed-dose ( FD ) combination therapy with inhaled glucocorticosteroids ( ICS ) and long acting beta ( 2 ) - adrenoceptor agonists ( LABA ) , many patients with asthma remain suboptimally controlled , based on the need for rescue therapy and rates of severe exacerbations .
	manualset3
262046	5	426200	7	NULL	NULL	NULL	NULL	asthma 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite aggressive fixed-dose ( FD ) combination therapy with inhaled glucocorticosteroids ( ICS ) and long acting beta ( 2 ) - adrenoceptor agonists ( LABA ) , many patients with asthma remain suboptimally controlled , based on the need for rescue therapy and rates of severe exacerbations .
	manualset3
262047	6	426200	7	NULL	NULL	NULL	NULL	 need 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite aggressive fixed-dose ( FD ) combination therapy with inhaled glucocorticosteroids ( ICS ) and long acting beta ( 2 ) - adrenoceptor agonists ( LABA ) , many patients with asthma remain suboptimally controlled , based on the need for rescue therapy and rates of severe exacerbations .
	manualset3
262048	7	426200	7	NULL	NULL	NULL	NULL	 rescue therapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite aggressive fixed-dose ( FD ) combination therapy with inhaled glucocorticosteroids ( ICS ) and long acting beta ( 2 ) - adrenoceptor agonists ( LABA ) , many patients with asthma remain suboptimally controlled , based on the need for rescue therapy and rates of severe exacerbations .
	manualset3
262049	8	426200	7	NULL	NULL	NULL	NULL	 rates 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite aggressive fixed-dose ( FD ) combination therapy with inhaled glucocorticosteroids ( ICS ) and long acting beta ( 2 ) - adrenoceptor agonists ( LABA ) , many patients with asthma remain suboptimally controlled , based on the need for rescue therapy and rates of severe exacerbations .
	manualset3
262050	9	426200	7	NULL	NULL	NULL	NULL	severe exacerbations 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite aggressive fixed-dose ( FD ) combination therapy with inhaled glucocorticosteroids ( ICS ) and long acting beta ( 2 ) - adrenoceptor agonists ( LABA ) , many patients with asthma remain suboptimally controlled , based on the need for rescue therapy and rates of severe exacerbations .
	manualset3
262051	1	426201	7	NULL	NULL	NULL	NULL	 conservation 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite conservation of peptide-binding specificity in HLA-E and Qa-1 , cross-species tetramer-staining experiments demonstrated that the interaction surfaces on CD94/NKG2 and the class Ib ligands have diverged between primates and rodents .
	manualset3
262052	2	426201	7	NULL	NULL	NULL	NULL	peptide-binding specificity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite conservation of peptide-binding specificity in HLA-E and Qa-1 , cross-species tetramer-staining experiments demonstrated that the interaction surfaces on CD94/NKG2 and the class Ib ligands have diverged between primates and rodents .
	manualset3
262053	3	426201	7	NULL	NULL	NULL	NULL	HLA-E	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite conservation of peptide-binding specificity in HLA-E and Qa-1 , cross-species tetramer-staining experiments demonstrated that the interaction surfaces on CD94/NKG2 and the class Ib ligands have diverged between primates and rodents .
	manualset3
262054	4	426201	7	NULL	NULL	NULL	NULL	Qa-1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite conservation of peptide-binding specificity in HLA-E and Qa-1 , cross-species tetramer-staining experiments demonstrated that the interaction surfaces on CD94/NKG2 and the class Ib ligands have diverged between primates and rodents .
	manualset3
262055	5	426201	7	NULL	NULL	NULL	NULL	cross-species tetramer-staining experiments	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite conservation of peptide-binding specificity in HLA-E and Qa-1 , cross-species tetramer-staining experiments demonstrated that the interaction surfaces on CD94/NKG2 and the class Ib ligands have diverged between primates and rodents .
	manualset3
262056	6	426201	7	NULL	NULL	NULL	NULL	interaction surfaces	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite conservation of peptide-binding specificity in HLA-E and Qa-1 , cross-species tetramer-staining experiments demonstrated that the interaction surfaces on CD94/NKG2 and the class Ib ligands have diverged between primates and rodents .
	manualset3
262057	7	426201	7	NULL	NULL	NULL	NULL	CD94/NKG2	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite conservation of peptide-binding specificity in HLA-E and Qa-1 , cross-species tetramer-staining experiments demonstrated that the interaction surfaces on CD94/NKG2 and the class Ib ligands have diverged between primates and rodents .
	manualset3
262058	8	426201	7	NULL	NULL	NULL	NULL	class Ib ligands	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite conservation of peptide-binding specificity in HLA-E and Qa-1 , cross-species tetramer-staining experiments demonstrated that the interaction surfaces on CD94/NKG2 and the class Ib ligands have diverged between primates and rodents .
	manualset3
262059	9	426201	7	NULL	NULL	NULL	NULL	primates	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite conservation of peptide-binding specificity in HLA-E and Qa-1 , cross-species tetramer-staining experiments demonstrated that the interaction surfaces on CD94/NKG2 and the class Ib ligands have diverged between primates and rodents .
	manualset3
262060	10	426201	7	NULL	NULL	NULL	NULL	rodents	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite conservation of peptide-binding specificity in HLA-E and Qa-1 , cross-species tetramer-staining experiments demonstrated that the interaction surfaces on CD94/NKG2 and the class Ib ligands have diverged between primates and rodents .
	manualset3
262061	1	426202	7	NULL	NULL	NULL	NULL	conservative treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite conservative treatment the fistula did not close spontaneously .
	manualset3
262062	2	426202	7	NULL	NULL	NULL	NULL	fistula	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite conservative treatment the fistula did not close spontaneously .
	manualset3
262063	1	426203	7	NULL	NULL	NULL	NULL	continuation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite continuation of CRH infusion , the inhibitory effect disappeared and plasma LH increased to similar levels as in controls at corresponding points of time of the LH surge .
	manualset3
262064	2	426203	7	NULL	NULL	NULL	NULL	CRH infusion	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite continuation of CRH infusion , the inhibitory effect disappeared and plasma LH increased to similar levels as in controls at corresponding points of time of the LH surge .
	manualset3
262065	3	426203	7	NULL	NULL	NULL	NULL	inhibitory effect	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite continuation of CRH infusion , the inhibitory effect disappeared and plasma LH increased to similar levels as in controls at corresponding points of time of the LH surge .
	manualset3
262066	4	426203	7	NULL	NULL	NULL	NULL	 plasma LH	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite continuation of CRH infusion , the inhibitory effect disappeared and plasma LH increased to similar levels as in controls at corresponding points of time of the LH surge .
	manualset3
262067	5	426203	7	NULL	NULL	NULL	NULL	 similar levels	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite continuation of CRH infusion , the inhibitory effect disappeared and plasma LH increased to similar levels as in controls at corresponding points of time of the LH surge .
	manualset3
262068	6	426203	7	NULL	NULL	NULL	NULL	controls	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite continuation of CRH infusion , the inhibitory effect disappeared and plasma LH increased to similar levels as in controls at corresponding points of time of the LH surge .
	manualset3
262069	7	426203	7	NULL	NULL	NULL	NULL	points of time	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite continuation of CRH infusion , the inhibitory effect disappeared and plasma LH increased to similar levels as in controls at corresponding points of time of the LH surge .
	manualset3
262070	8	426203	7	NULL	NULL	NULL	NULL	LH surge	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite continuation of CRH infusion , the inhibitory effect disappeared and plasma LH increased to similar levels as in controls at corresponding points of time of the LH surge .
	manualset3
262071	1	426204	7	NULL	NULL	NULL	NULL	high growth rates	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite high growth rates and associated problems , population growth does not present the major threat in Africa .
	manualset3
262072	2	426204	7	NULL	NULL	NULL	NULL	associated problems	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite high growth rates and associated problems , population growth does not present the major threat in Africa .
	manualset3
262073	3	426204	7	NULL	NULL	NULL	NULL	population growth	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite high growth rates and associated problems , population growth does not present the major threat in Africa .
	manualset3
262074	4	426204	7	NULL	NULL	NULL	NULL	major threat	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite high growth rates and associated problems , population growth does not present the major threat in Africa .
	manualset3
262075	5	426204	7	NULL	NULL	NULL	NULL	Africa 	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite high growth rates and associated problems , population growth does not present the major threat in Africa .
	manualset3
262076	1	426205	7	NULL	NULL	NULL	NULL	increased 5-HT metabolism	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite increased 5-HT metabolism , brain 5-HT release in rats with a portacaval shunt ( PCS ) seems to be unaltered .
	manualset3
262077	2	426205	7	NULL	NULL	NULL	NULL	brain 5-HT release	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite increased 5-HT metabolism , brain 5-HT release in rats with a portacaval shunt ( PCS ) seems to be unaltered .
	manualset3
262078	3	426205	7	NULL	NULL	NULL	NULL	 rats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite increased 5-HT metabolism , brain 5-HT release in rats with a portacaval shunt ( PCS ) seems to be unaltered .
	manualset3
262079	4	426205	7	NULL	NULL	NULL	NULL	portacaval shunt ( PCS )	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite increased 5-HT metabolism , brain 5-HT release in rats with a portacaval shunt ( PCS ) seems to be unaltered .
	manualset3
262080	1	426206	7	NULL	NULL	NULL	NULL	 iron influx	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite increased iron influx in inhibited cells , only 2-4 % of total incoming iron was diverted into ferritin .
	manualset3
262081	2	426206	7	NULL	NULL	NULL	NULL	cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite increased iron influx in inhibited cells , only 2-4 % of total incoming iron was diverted into ferritin .
	manualset3
262082	3	426206	7	NULL	NULL	NULL	NULL	2-4 %	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite increased iron influx in inhibited cells , only 2-4 % of total incoming iron was diverted into ferritin .
	manualset3
262083	4	426206	7	NULL	NULL	NULL	NULL	total incoming iron	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite increased iron influx in inhibited cells , only 2-4 % of total incoming iron was diverted into ferritin .
	manualset3
262084	5	426206	7	NULL	NULL	NULL	NULL	 ferritin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite increased iron influx in inhibited cells , only 2-4 % of total incoming iron was diverted into ferritin .
	manualset3
262085	1	426207	7	NULL	NULL	NULL	NULL	 high level	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite its high level of attenuation , the E5 3 ' deletion mutant remained highly immunogenic and intraperitoneal ( ip ) inoculation of 10 PFU induced complete protection in Swiss mice against subsequent challenge with 2000 ip LD50 of the wild-type LGT TP21 .
	manualset3
262086	2	426207	7	NULL	NULL	NULL	NULL	attenuation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite its high level of attenuation , the E5 3 ' deletion mutant remained highly immunogenic and intraperitoneal ( ip ) inoculation of 10 PFU induced complete protection in Swiss mice against subsequent challenge with 2000 ip LD50 of the wild-type LGT TP21 .
	manualset3
262087	3	426207	7	NULL	NULL	NULL	NULL	E5 3 ' deletion mutant	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite its high level of attenuation , the E5 3 ' deletion mutant remained highly immunogenic and intraperitoneal ( ip ) inoculation of 10 PFU induced complete protection in Swiss mice against subsequent challenge with 2000 ip LD50 of the wild-type LGT TP21 .
	manualset3
262088	4	426207	7	NULL	NULL	NULL	NULL	 intraperitoneal ( ip ) inoculation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite its high level of attenuation , the E5 3 ' deletion mutant remained highly immunogenic and intraperitoneal ( ip ) inoculation of 10 PFU induced complete protection in Swiss mice against subsequent challenge with 2000 ip LD50 of the wild-type LGT TP21 .
	manualset3
262089	5	426207	7	NULL	NULL	NULL	NULL	10 PFU 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite its high level of attenuation , the E5 3 ' deletion mutant remained highly immunogenic and intraperitoneal ( ip ) inoculation of 10 PFU induced complete protection in Swiss mice against subsequent challenge with 2000 ip LD50 of the wild-type LGT TP21 .
	manualset3
262090	6	426207	7	NULL	NULL	NULL	NULL	complete protection	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite its high level of attenuation , the E5 3 ' deletion mutant remained highly immunogenic and intraperitoneal ( ip ) inoculation of 10 PFU induced complete protection in Swiss mice against subsequent challenge with 2000 ip LD50 of the wild-type LGT TP21 .
	manualset3
262091	7	426207	7	NULL	NULL	NULL	NULL	Swiss mice	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite its high level of attenuation , the E5 3 ' deletion mutant remained highly immunogenic and intraperitoneal ( ip ) inoculation of 10 PFU induced complete protection in Swiss mice against subsequent challenge with 2000 ip LD50 of the wild-type LGT TP21 .
	manualset3
262092	8	426207	7	NULL	NULL	NULL	NULL	challenge	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite its high level of attenuation , the E5 3 ' deletion mutant remained highly immunogenic and intraperitoneal ( ip ) inoculation of 10 PFU induced complete protection in Swiss mice against subsequent challenge with 2000 ip LD50 of the wild-type LGT TP21 .
	manualset3
262093	9	426207	7	NULL	NULL	NULL	NULL	2000 ip LD50 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite its high level of attenuation , the E5 3 ' deletion mutant remained highly immunogenic and intraperitoneal ( ip ) inoculation of 10 PFU induced complete protection in Swiss mice against subsequent challenge with 2000 ip LD50 of the wild-type LGT TP21 .
	manualset3
262094	10	426207	7	NULL	NULL	NULL	NULL	 wild-type LGT TP21	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite its high level of attenuation , the E5 3 ' deletion mutant remained highly immunogenic and intraperitoneal ( ip ) inoculation of 10 PFU induced complete protection in Swiss mice against subsequent challenge with 2000 ip LD50 of the wild-type LGT TP21 .
	manualset3
262095	1	426208	7	NULL	NULL	NULL	NULL	lip service	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite lip service paid to prescriptive eclecticism , most graduate programs socialize their students into delimited schools of thought .
	manualset3
262096	2	426208	7	NULL	NULL	NULL	NULL	prescriptive eclecticism	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite lip service paid to prescriptive eclecticism , most graduate programs socialize their students into delimited schools of thought .
	manualset3
262097	3	426208	7	NULL	NULL	NULL	NULL	graduate programs	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite lip service paid to prescriptive eclecticism , most graduate programs socialize their students into delimited schools of thought .
	manualset3
262098	4	426208	7	NULL	NULL	NULL	NULL	students 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite lip service paid to prescriptive eclecticism , most graduate programs socialize their students into delimited schools of thought .
	manualset3
262099	5	426208	7	NULL	NULL	NULL	NULL	schools of thought	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite lip service paid to prescriptive eclecticism , most graduate programs socialize their students into delimited schools of thought .
	manualset3
262100	1	426209	7	NULL	NULL	NULL	NULL	multiple proofs 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite multiple proofs of beneficial effects of aldosterone receptor blockers on clinical course of CHF wide use of spironolactone and eplerenone is not recommended because of multiple communications about life threatening hyperkalemia .
	manualset3
262101	2	426209	7	NULL	NULL	NULL	NULL	beneficial effects	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite multiple proofs of beneficial effects of aldosterone receptor blockers on clinical course of CHF wide use of spironolactone and eplerenone is not recommended because of multiple communications about life threatening hyperkalemia .
	manualset3
262102	3	426209	7	NULL	NULL	NULL	NULL	 aldosterone receptor blockers	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite multiple proofs of beneficial effects of aldosterone receptor blockers on clinical course of CHF wide use of spironolactone and eplerenone is not recommended because of multiple communications about life threatening hyperkalemia .
	manualset3
262103	4	426209	7	NULL	NULL	NULL	NULL	clinical course	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite multiple proofs of beneficial effects of aldosterone receptor blockers on clinical course of CHF wide use of spironolactone and eplerenone is not recommended because of multiple communications about life threatening hyperkalemia .
	manualset3
262104	5	426209	7	NULL	NULL	NULL	NULL	CHF	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite multiple proofs of beneficial effects of aldosterone receptor blockers on clinical course of CHF wide use of spironolactone and eplerenone is not recommended because of multiple communications about life threatening hyperkalemia .
	manualset3
262105	6	426209	7	NULL	NULL	NULL	NULL	use	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite multiple proofs of beneficial effects of aldosterone receptor blockers on clinical course of CHF wide use of spironolactone and eplerenone is not recommended because of multiple communications about life threatening hyperkalemia .
	manualset3
262106	7	426209	7	NULL	NULL	NULL	NULL	spironolactone	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite multiple proofs of beneficial effects of aldosterone receptor blockers on clinical course of CHF wide use of spironolactone and eplerenone is not recommended because of multiple communications about life threatening hyperkalemia .
	manualset3
262107	8	426209	7	NULL	NULL	NULL	NULL	eplerenone	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite multiple proofs of beneficial effects of aldosterone receptor blockers on clinical course of CHF wide use of spironolactone and eplerenone is not recommended because of multiple communications about life threatening hyperkalemia .
	manualset3
262108	9	426209	7	NULL	NULL	NULL	NULL	multiple communications	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite multiple proofs of beneficial effects of aldosterone receptor blockers on clinical course of CHF wide use of spironolactone and eplerenone is not recommended because of multiple communications about life threatening hyperkalemia .
	manualset3
262109	10	426209	7	NULL	NULL	NULL	NULL	life threatening hyperkalemia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite multiple proofs of beneficial effects of aldosterone receptor blockers on clinical course of CHF wide use of spironolactone and eplerenone is not recommended because of multiple communications about life threatening hyperkalemia .
	manualset3
262110	1	426210	7	NULL	NULL	NULL	NULL	recent advances	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite recent advances in medical therapy , reperfusion strategies , implantable cardioverter-defibrillators and cardiac assist devices , ischemic heart disease is a frequent cause of morbidity and mortality worldwide .
	manualset3
262111	2	426210	7	NULL	NULL	NULL	NULL	medical therapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite recent advances in medical therapy , reperfusion strategies , implantable cardioverter-defibrillators and cardiac assist devices , ischemic heart disease is a frequent cause of morbidity and mortality worldwide .
	manualset3
262112	3	426210	7	NULL	NULL	NULL	NULL	reperfusion strategies 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite recent advances in medical therapy , reperfusion strategies , implantable cardioverter-defibrillators and cardiac assist devices , ischemic heart disease is a frequent cause of morbidity and mortality worldwide .
	manualset3
262113	4	426210	7	NULL	NULL	NULL	NULL	 implantable cardioverter-defibrillators 	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite recent advances in medical therapy , reperfusion strategies , implantable cardioverter-defibrillators and cardiac assist devices , ischemic heart disease is a frequent cause of morbidity and mortality worldwide .
	manualset3
262114	5	426210	7	NULL	NULL	NULL	NULL	cardiac assist devices	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite recent advances in medical therapy , reperfusion strategies , implantable cardioverter-defibrillators and cardiac assist devices , ischemic heart disease is a frequent cause of morbidity and mortality worldwide .
	manualset3
262115	6	426210	7	NULL	NULL	NULL	NULL	 ischemic heart disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite recent advances in medical therapy , reperfusion strategies , implantable cardioverter-defibrillators and cardiac assist devices , ischemic heart disease is a frequent cause of morbidity and mortality worldwide .
	manualset3
262116	7	426210	7	NULL	NULL	NULL	NULL	cause	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite recent advances in medical therapy , reperfusion strategies , implantable cardioverter-defibrillators and cardiac assist devices , ischemic heart disease is a frequent cause of morbidity and mortality worldwide .
	manualset3
262117	8	426210	7	NULL	NULL	NULL	NULL	morbidity 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite recent advances in medical therapy , reperfusion strategies , implantable cardioverter-defibrillators and cardiac assist devices , ischemic heart disease is a frequent cause of morbidity and mortality worldwide .
	manualset3
262118	9	426210	7	NULL	NULL	NULL	NULL	mortality	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite recent advances in medical therapy , reperfusion strategies , implantable cardioverter-defibrillators and cardiac assist devices , ischemic heart disease is a frequent cause of morbidity and mortality worldwide .
	manualset3
262413	1	426211	7	NULL	NULL	NULL	NULL	New developments 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( New developments in the etiologic diagnosis and study of the clinic and pathogenesis of tick-borne encephalitis ) .
	manualset3
262414	2	426211	7	NULL	NULL	NULL	NULL	etiologic diagnosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( New developments in the etiologic diagnosis and study of the clinic and pathogenesis of tick-borne encephalitis ) .
	manualset3
262415	3	426211	7	NULL	NULL	NULL	NULL	study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( New developments in the etiologic diagnosis and study of the clinic and pathogenesis of tick-borne encephalitis ) .
	manualset3
262417	4	426211	7	NULL	NULL	NULL	NULL	clinic	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( New developments in the etiologic diagnosis and study of the clinic and pathogenesis of tick-borne encephalitis ) .
	manualset3
262418	5	426211	7	NULL	NULL	NULL	NULL	pathogenesis 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( New developments in the etiologic diagnosis and study of the clinic and pathogenesis of tick-borne encephalitis ) .
	manualset3
262420	6	426211	7	NULL	NULL	NULL	NULL	tick-borne encephalitis 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( New developments in the etiologic diagnosis and study of the clinic and pathogenesis of tick-borne encephalitis ) .
	manualset3
262424	1	426212	7	NULL	NULL	NULL	NULL	lower subjective well being	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite significantly lower subjective well being and health than both the general population and HT group , the environmentally annoyed subjects had lower health care costs than the hypertension group .
	manualset3
262425	2	426212	7	NULL	NULL	NULL	NULL	health	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite significantly lower subjective well being and health than both the general population and HT group , the environmentally annoyed subjects had lower health care costs than the hypertension group .
	manualset3
262426	3	426212	7	NULL	NULL	NULL	NULL	general population	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite significantly lower subjective well being and health than both the general population and HT group , the environmentally annoyed subjects had lower health care costs than the hypertension group .
	manualset3
262428	4	426212	7	NULL	NULL	NULL	NULL	 HT group	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite significantly lower subjective well being and health than both the general population and HT group , the environmentally annoyed subjects had lower health care costs than the hypertension group .
	manualset3
262429	5	426212	7	NULL	NULL	NULL	NULL	environmentally annoyed subjects	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite significantly lower subjective well being and health than both the general population and HT group , the environmentally annoyed subjects had lower health care costs than the hypertension group .
	manualset3
262430	6	426212	7	NULL	NULL	NULL	NULL	health care costs	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite significantly lower subjective well being and health than both the general population and HT group , the environmentally annoyed subjects had lower health care costs than the hypertension group .
	manualset3
262432	7	426212	7	NULL	NULL	NULL	NULL	hypertension group	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite significantly lower subjective well being and health than both the general population and HT group , the environmentally annoyed subjects had lower health care costs than the hypertension group .
	manualset3
262456	1	426213	7	NULL	NULL	NULL	NULL	small changes	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite small changes in the quantitative results caused by nonspecific variation and boosting , the diagnostic result of the QFT-GIT was reliable .
	manualset3
262459	2	426213	7	NULL	NULL	NULL	NULL	quantitative results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite small changes in the quantitative results caused by nonspecific variation and boosting , the diagnostic result of the QFT-GIT was reliable .
	manualset3
262460	3	426213	7	NULL	NULL	NULL	NULL	nonspecific variation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite small changes in the quantitative results caused by nonspecific variation and boosting , the diagnostic result of the QFT-GIT was reliable .
	manualset3
262461	4	426213	7	NULL	NULL	NULL	NULL	boosting	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite small changes in the quantitative results caused by nonspecific variation and boosting , the diagnostic result of the QFT-GIT was reliable .
	manualset3
262463	5	426213	7	NULL	NULL	NULL	NULL	diagnostic result	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite small changes in the quantitative results caused by nonspecific variation and boosting , the diagnostic result of the QFT-GIT was reliable .
	manualset3
262469	6	426213	7	NULL	NULL	NULL	NULL	QFT-GIT 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite small changes in the quantitative results caused by nonspecific variation and boosting , the diagnostic result of the QFT-GIT was reliable .
	manualset3
262474	1	426214	7	NULL	NULL	NULL	NULL	 social differences	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite social and cultural differences between street youth in developing countries versus homeless youth in developed countries , the predictors and correlates of homelessness are similar among youth .
	manualset3
262476	2	426214	7	NULL	NULL	NULL	NULL	cultural differences	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite social and cultural differences between street youth in developing countries versus homeless youth in developed countries , the predictors and correlates of homelessness are similar among youth .
	manualset3
262478	3	426214	7	NULL	NULL	NULL	NULL	street youth	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite social and cultural differences between street youth in developing countries versus homeless youth in developed countries , the predictors and correlates of homelessness are similar among youth .
	manualset3
262490	4	426214	7	NULL	NULL	NULL	NULL	developing countries	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite social and cultural differences between street youth in developing countries versus homeless youth in developed countries , the predictors and correlates of homelessness are similar among youth .
	manualset3
262491	5	426214	7	NULL	NULL	NULL	NULL	 homeless youth	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite social and cultural differences between street youth in developing countries versus homeless youth in developed countries , the predictors and correlates of homelessness are similar among youth .
	manualset3
262493	6	426214	7	NULL	NULL	NULL	NULL	developed countries	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite social and cultural differences between street youth in developing countries versus homeless youth in developed countries , the predictors and correlates of homelessness are similar among youth .
	manualset3
262495	7	426214	7	NULL	NULL	NULL	NULL	 predictors	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite social and cultural differences between street youth in developing countries versus homeless youth in developed countries , the predictors and correlates of homelessness are similar among youth .
	manualset3
262496	8	426214	7	NULL	NULL	NULL	NULL	homelessness	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite social and cultural differences between street youth in developing countries versus homeless youth in developed countries , the predictors and correlates of homelessness are similar among youth .
	manualset3
262502	9	426214	7	NULL	NULL	NULL	NULL	 youth	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite social and cultural differences between street youth in developing countries versus homeless youth in developed countries , the predictors and correlates of homelessness are similar among youth .
	manualset3
262507	1	426215	7	NULL	NULL	NULL	NULL	XBP1 splicing	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the XBP1 splicing and PERK gene expression induced by DUGV , no ER-stress and apoptosis crosstalk was observed .
	manualset3
262509	2	426215	7	NULL	NULL	NULL	NULL	PERK gene expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the XBP1 splicing and PERK gene expression induced by DUGV , no ER-stress and apoptosis crosstalk was observed .
	manualset3
262513	3	426215	7	NULL	NULL	NULL	NULL	DUGV	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the XBP1 splicing and PERK gene expression induced by DUGV , no ER-stress and apoptosis crosstalk was observed .
	manualset3
262514	4	426215	7	NULL	NULL	NULL	NULL	ER-stress	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the XBP1 splicing and PERK gene expression induced by DUGV , no ER-stress and apoptosis crosstalk was observed .
	manualset3
262515	5	426215	7	NULL	NULL	NULL	NULL	apoptosis crosstalk	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the XBP1 splicing and PERK gene expression induced by DUGV , no ER-stress and apoptosis crosstalk was observed .
	manualset3
262517	1	426216	7	NULL	NULL	NULL	NULL	 absence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the absence of apparent genomic activation mechanisms accounting for overexpression , clinical study of IGF1R-directed therapies in pediatric WT GIST is warranted .
	manualset3
262518	2	426216	7	NULL	NULL	NULL	NULL	genomic activation mechanisms	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the absence of apparent genomic activation mechanisms accounting for overexpression , clinical study of IGF1R-directed therapies in pediatric WT GIST is warranted .
	manualset3
262520	3	426216	7	NULL	NULL	NULL	NULL	overexpression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the absence of apparent genomic activation mechanisms accounting for overexpression , clinical study of IGF1R-directed therapies in pediatric WT GIST is warranted .
	manualset3
262522	4	426216	7	NULL	NULL	NULL	NULL	clinical study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the absence of apparent genomic activation mechanisms accounting for overexpression , clinical study of IGF1R-directed therapies in pediatric WT GIST is warranted .
	manualset3
262523	5	426216	7	NULL	NULL	NULL	NULL	 IGF1R-directed therapies	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the absence of apparent genomic activation mechanisms accounting for overexpression , clinical study of IGF1R-directed therapies in pediatric WT GIST is warranted .
	manualset3
262528	6	426216	7	NULL	NULL	NULL	NULL	pediatric WT GIST	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the absence of apparent genomic activation mechanisms accounting for overexpression , clinical study of IGF1R-directed therapies in pediatric WT GIST is warranted .
	manualset3
262533	1	426217	7	NULL	NULL	NULL	NULL	absence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the absence of the signal peptide sequence necessary for protein secretion , annexin 1 was released in the keratinocyte culture medium .
	manualset3
262535	2	426217	7	NULL	NULL	NULL	NULL	signal peptide sequence	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the absence of the signal peptide sequence necessary for protein secretion , annexin 1 was released in the keratinocyte culture medium .
	manualset3
262536	3	426217	7	NULL	NULL	NULL	NULL	protein secretion	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the absence of the signal peptide sequence necessary for protein secretion , annexin 1 was released in the keratinocyte culture medium .
	manualset3
262537	4	426217	7	NULL	NULL	NULL	NULL	 annexin 1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the absence of the signal peptide sequence necessary for protein secretion , annexin 1 was released in the keratinocyte culture medium .
	manualset3
262538	5	426217	7	NULL	NULL	NULL	NULL	keratinocyte culture medium	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the absence of the signal peptide sequence necessary for protein secretion , annexin 1 was released in the keratinocyte culture medium .
	manualset3
262541	1	426218	7	NULL	NULL	NULL	NULL	achievement 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the achievement of continence , the rectosphincteric reflexes following treatment continued to be abnormal in every case .
	manualset3
262542	2	426218	7	NULL	NULL	NULL	NULL	continence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the achievement of continence , the rectosphincteric reflexes following treatment continued to be abnormal in every case .
	manualset3
262543	3	426218	7	NULL	NULL	NULL	NULL	rectosphincteric reflexes	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the achievement of continence , the rectosphincteric reflexes following treatment continued to be abnormal in every case .
	manualset3
262544	4	426218	7	NULL	NULL	NULL	NULL	treatment 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the achievement of continence , the rectosphincteric reflexes following treatment continued to be abnormal in every case .
	manualset3
262545	5	426218	7	NULL	NULL	NULL	NULL	abnormal 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the achievement of continence , the rectosphincteric reflexes following treatment continued to be abnormal in every case .
	manualset3
262546	6	426218	7	NULL	NULL	NULL	NULL	case	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the achievement of continence , the rectosphincteric reflexes following treatment continued to be abnormal in every case .
	manualset3
262547	1	426219	7	NULL	NULL	NULL	NULL	decrease 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the decrease in Pfr central , however , Vmax failed to increase after atropine because of altered bronchial area pressure ( BAP ) behavior at the CP site .
	manualset3
262548	2	426219	7	NULL	NULL	NULL	NULL	Pfr central	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the decrease in Pfr central , however , Vmax failed to increase after atropine because of altered bronchial area pressure ( BAP ) behavior at the CP site .
	manualset3
262549	3	426219	7	NULL	NULL	NULL	NULL	Vmax	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the decrease in Pfr central , however , Vmax failed to increase after atropine because of altered bronchial area pressure ( BAP ) behavior at the CP site .
	manualset3
262550	4	426219	7	NULL	NULL	NULL	NULL	atropine	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the decrease in Pfr central , however , Vmax failed to increase after atropine because of altered bronchial area pressure ( BAP ) behavior at the CP site .
	manualset3
262551	5	426219	7	NULL	NULL	NULL	NULL	bronchial area pressure ( BAP ) behavior	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the decrease in Pfr central , however , Vmax failed to increase after atropine because of altered bronchial area pressure ( BAP ) behavior at the CP site .
	manualset3
262552	6	426219	7	NULL	NULL	NULL	NULL	CP site	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the decrease in Pfr central , however , Vmax failed to increase after atropine because of altered bronchial area pressure ( BAP ) behavior at the CP site .
	manualset3
262553	1	426220	7	NULL	NULL	NULL	NULL	 economic importance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the enormous economic and ecological importance of marine organisms , the spatial scales of adaptation and biocomplexity remain largely unknown .
	manualset3
262554	2	426220	7	NULL	NULL	NULL	NULL	ecological importance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the enormous economic and ecological importance of marine organisms , the spatial scales of adaptation and biocomplexity remain largely unknown .
	manualset3
262555	3	426220	7	NULL	NULL	NULL	NULL	marine organisms	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the enormous economic and ecological importance of marine organisms , the spatial scales of adaptation and biocomplexity remain largely unknown .
	manualset3
262556	4	426220	7	NULL	NULL	NULL	NULL	spatial scales	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the enormous economic and ecological importance of marine organisms , the spatial scales of adaptation and biocomplexity remain largely unknown .
	manualset3
262557	5	426220	7	NULL	NULL	NULL	NULL	adaptation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the enormous economic and ecological importance of marine organisms , the spatial scales of adaptation and biocomplexity remain largely unknown .
	manualset3
262558	6	426220	7	NULL	NULL	NULL	NULL	biocomplexity	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the enormous economic and ecological importance of marine organisms , the spatial scales of adaptation and biocomplexity remain largely unknown .
	manualset3
262696	1	426221	7	NULL	NULL	NULL	NULL	L-carnosine-related peptidomimetics N-acetylcarnosine ( N-acetyl-beta-alanyl-L-histidine ) ( NAC )	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the fact that L-carnosine-related peptidomimetics N-acetylcarnosine ( N-acetyl-beta-alanyl-L-histidine ) ( NAC ) and carcinine ( beta-alanylhistamine ) are metabolically related to L-carnosine and have been demonstrated to occur in tissues of many vertebrates , including humans , these compounds were shown resistant toward enzymatic hydrolysis .
	manualset3
262697	2	426221	7	NULL	NULL	NULL	NULL	 carcinine ( beta-alanylhistamine )	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the fact that L-carnosine-related peptidomimetics N-acetylcarnosine ( N-acetyl-beta-alanyl-L-histidine ) ( NAC ) and carcinine ( beta-alanylhistamine ) are metabolically related to L-carnosine and have been demonstrated to occur in tissues of many vertebrates , including humans , these compounds were shown resistant toward enzymatic hydrolysis .
	manualset3
262698	3	426221	7	NULL	NULL	NULL	NULL	 L-carnosine	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the fact that L-carnosine-related peptidomimetics N-acetylcarnosine ( N-acetyl-beta-alanyl-L-histidine ) ( NAC ) and carcinine ( beta-alanylhistamine ) are metabolically related to L-carnosine and have been demonstrated to occur in tissues of many vertebrates , including humans , these compounds were shown resistant toward enzymatic hydrolysis .
	manualset3
262699	4	426221	7	NULL	NULL	NULL	NULL	tissues 	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the fact that L-carnosine-related peptidomimetics N-acetylcarnosine ( N-acetyl-beta-alanyl-L-histidine ) ( NAC ) and carcinine ( beta-alanylhistamine ) are metabolically related to L-carnosine and have been demonstrated to occur in tissues of many vertebrates , including humans , these compounds were shown resistant toward enzymatic hydrolysis .
	manualset3
262700	5	426221	7	NULL	NULL	NULL	NULL	 vertebrates	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the fact that L-carnosine-related peptidomimetics N-acetylcarnosine ( N-acetyl-beta-alanyl-L-histidine ) ( NAC ) and carcinine ( beta-alanylhistamine ) are metabolically related to L-carnosine and have been demonstrated to occur in tissues of many vertebrates , including humans , these compounds were shown resistant toward enzymatic hydrolysis .
	manualset3
262701	6	426221	7	NULL	NULL	NULL	NULL	humans 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the fact that L-carnosine-related peptidomimetics N-acetylcarnosine ( N-acetyl-beta-alanyl-L-histidine ) ( NAC ) and carcinine ( beta-alanylhistamine ) are metabolically related to L-carnosine and have been demonstrated to occur in tissues of many vertebrates , including humans , these compounds were shown resistant toward enzymatic hydrolysis .
	manualset3
262702	7	426221	7	NULL	NULL	NULL	NULL	compounds	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the fact that L-carnosine-related peptidomimetics N-acetylcarnosine ( N-acetyl-beta-alanyl-L-histidine ) ( NAC ) and carcinine ( beta-alanylhistamine ) are metabolically related to L-carnosine and have been demonstrated to occur in tissues of many vertebrates , including humans , these compounds were shown resistant toward enzymatic hydrolysis .
	manualset3
262703	8	426221	7	NULL	NULL	NULL	NULL	enzymatic hydrolysis	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the fact that L-carnosine-related peptidomimetics N-acetylcarnosine ( N-acetyl-beta-alanyl-L-histidine ) ( NAC ) and carcinine ( beta-alanylhistamine ) are metabolically related to L-carnosine and have been demonstrated to occur in tissues of many vertebrates , including humans , these compounds were shown resistant toward enzymatic hydrolysis .
	manualset3
262704	1	426222	7	NULL	NULL	NULL	NULL	NSC	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the fact that NSC and antibody-dependent cellular cytotoxicity ( ADCC ) are both mediated through neutrophil Fc gamma R and require the activation of the respiratory burst , the cytolytic mechanisms involved in each case appear to be different .
	manualset3
262705	2	426222	7	NULL	NULL	NULL	NULL	antibody-dependent cellular cytotoxicity ( ADCC )	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the fact that NSC and antibody-dependent cellular cytotoxicity ( ADCC ) are both mediated through neutrophil Fc gamma R and require the activation of the respiratory burst , the cytolytic mechanisms involved in each case appear to be different .
	manualset3
262706	3	426222	7	NULL	NULL	NULL	NULL	neutrophil Fc gamma R	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the fact that NSC and antibody-dependent cellular cytotoxicity ( ADCC ) are both mediated through neutrophil Fc gamma R and require the activation of the respiratory burst , the cytolytic mechanisms involved in each case appear to be different .
	manualset3
262707	4	426222	7	NULL	NULL	NULL	NULL	activation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the fact that NSC and antibody-dependent cellular cytotoxicity ( ADCC ) are both mediated through neutrophil Fc gamma R and require the activation of the respiratory burst , the cytolytic mechanisms involved in each case appear to be different .
	manualset3
262708	5	426222	7	NULL	NULL	NULL	NULL	respiratory burst	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the fact that NSC and antibody-dependent cellular cytotoxicity ( ADCC ) are both mediated through neutrophil Fc gamma R and require the activation of the respiratory burst , the cytolytic mechanisms involved in each case appear to be different .
	manualset3
262709	6	426222	7	NULL	NULL	NULL	NULL	cytolytic mechanisms 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the fact that NSC and antibody-dependent cellular cytotoxicity ( ADCC ) are both mediated through neutrophil Fc gamma R and require the activation of the respiratory burst , the cytolytic mechanisms involved in each case appear to be different .
	manualset3
262710	7	426222	7	NULL	NULL	NULL	NULL	case	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the fact that NSC and antibody-dependent cellular cytotoxicity ( ADCC ) are both mediated through neutrophil Fc gamma R and require the activation of the respiratory burst , the cytolytic mechanisms involved in each case appear to be different .
	manualset3
262711	1	426223	7	NULL	NULL	NULL	NULL	segmentation results 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the fact that segmentation results show good efficiency , the time is a key variable that has always to be optimized in a medical context .
	manualset3
262712	2	426223	7	NULL	NULL	NULL	NULL	 good efficiency	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the fact that segmentation results show good efficiency , the time is a key variable that has always to be optimized in a medical context .
	manualset3
262713	3	426223	7	NULL	NULL	NULL	NULL	time	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the fact that segmentation results show good efficiency , the time is a key variable that has always to be optimized in a medical context .
	manualset3
262714	4	426223	7	NULL	NULL	NULL	NULL	key variable	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the fact that segmentation results show good efficiency , the time is a key variable that has always to be optimized in a medical context .
	manualset3
262715	5	426223	7	NULL	NULL	NULL	NULL	medical context	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the fact that segmentation results show good efficiency , the time is a key variable that has always to be optimized in a medical context .
	manualset3
262716	1	426224	7	NULL	NULL	NULL	NULL	contribution	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the important contribution given by Italian clinical researchers to the demonstration that less radical surgery can be as good as more radical procedures , still a substantial proportion of breast cancer patients are treated too aggressively .
	manualset3
262717	2	426224	7	NULL	NULL	NULL	NULL	Italian clinical researchers	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the important contribution given by Italian clinical researchers to the demonstration that less radical surgery can be as good as more radical procedures , still a substantial proportion of breast cancer patients are treated too aggressively .
	manualset3
262718	3	426224	7	NULL	NULL	NULL	NULL	demonstration	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the important contribution given by Italian clinical researchers to the demonstration that less radical surgery can be as good as more radical procedures , still a substantial proportion of breast cancer patients are treated too aggressively .
	manualset3
262719	4	426224	7	NULL	NULL	NULL	NULL	radical surgery	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the important contribution given by Italian clinical researchers to the demonstration that less radical surgery can be as good as more radical procedures , still a substantial proportion of breast cancer patients are treated too aggressively .
	manualset3
262720	5	426224	7	NULL	NULL	NULL	NULL	radical procedures	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the important contribution given by Italian clinical researchers to the demonstration that less radical surgery can be as good as more radical procedures , still a substantial proportion of breast cancer patients are treated too aggressively .
	manualset3
262721	6	426224	7	NULL	NULL	NULL	NULL	substantial proportion 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the important contribution given by Italian clinical researchers to the demonstration that less radical surgery can be as good as more radical procedures , still a substantial proportion of breast cancer patients are treated too aggressively .
	manualset3
262722	7	426224	7	NULL	NULL	NULL	NULL	breast cancer patients 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the important contribution given by Italian clinical researchers to the demonstration that less radical surgery can be as good as more radical procedures , still a substantial proportion of breast cancer patients are treated too aggressively .
	manualset3
262723	1	426225	7	NULL	NULL	NULL	NULL	 long lasting research	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the long lasting research the ideal method of reconstructing the ACL has not been found so far .
	manualset3
262724	2	426225	7	NULL	NULL	NULL	NULL	ideal method	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the long lasting research the ideal method of reconstructing the ACL has not been found so far .
	manualset3
262725	3	426225	7	NULL	NULL	NULL	NULL	ACL	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the long lasting research the ideal method of reconstructing the ACL has not been found so far .
	manualset3
262726	1	426226	7	NULL	NULL	NULL	NULL	marked solubilization	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the marked solubilization of type X collagen upon administration of beta APN , a substantial proportion remained tissue-bound and could only be extracted by employing proteolytic digestion followed by disulphide bond reduction .
	manualset3
262727	2	426226	7	NULL	NULL	NULL	NULL	type X collagen	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the marked solubilization of type X collagen upon administration of beta APN , a substantial proportion remained tissue-bound and could only be extracted by employing proteolytic digestion followed by disulphide bond reduction .
	manualset3
262728	3	426226	7	NULL	NULL	NULL	NULL	administration	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the marked solubilization of type X collagen upon administration of beta APN , a substantial proportion remained tissue-bound and could only be extracted by employing proteolytic digestion followed by disulphide bond reduction .
	manualset3
262729	4	426226	7	NULL	NULL	NULL	NULL	beta APN	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the marked solubilization of type X collagen upon administration of beta APN , a substantial proportion remained tissue-bound and could only be extracted by employing proteolytic digestion followed by disulphide bond reduction .
	manualset3
262730	5	426226	7	NULL	NULL	NULL	NULL	 substantial proportion	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the marked solubilization of type X collagen upon administration of beta APN , a substantial proportion remained tissue-bound and could only be extracted by employing proteolytic digestion followed by disulphide bond reduction .
	manualset3
262731	6	426226	7	NULL	NULL	NULL	NULL	proteolytic digestion	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the marked solubilization of type X collagen upon administration of beta APN , a substantial proportion remained tissue-bound and could only be extracted by employing proteolytic digestion followed by disulphide bond reduction .
	manualset3
262732	7	426226	7	NULL	NULL	NULL	NULL	disulphide bond reduction	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the marked solubilization of type X collagen upon administration of beta APN , a substantial proportion remained tissue-bound and could only be extracted by employing proteolytic digestion followed by disulphide bond reduction .
	manualset3
262733	1	426227	7	NULL	NULL	NULL	NULL	ready access	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the ready access to the skin compared with solid internal organs , the challenges of cutaneous gene therapy are legion and many technical issues need to be surmounted to enable gene replacement or modification of gene expression to have a useful role in these disorders .
	manualset3
262734	2	426227	7	NULL	NULL	NULL	NULL	 skin	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the ready access to the skin compared with solid internal organs , the challenges of cutaneous gene therapy are legion and many technical issues need to be surmounted to enable gene replacement or modification of gene expression to have a useful role in these disorders .
	manualset3
262735	3	426227	7	NULL	NULL	NULL	NULL	 solid internal organs	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the ready access to the skin compared with solid internal organs , the challenges of cutaneous gene therapy are legion and many technical issues need to be surmounted to enable gene replacement or modification of gene expression to have a useful role in these disorders .
	manualset3
262736	4	426227	7	NULL	NULL	NULL	NULL	challenges	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the ready access to the skin compared with solid internal organs , the challenges of cutaneous gene therapy are legion and many technical issues need to be surmounted to enable gene replacement or modification of gene expression to have a useful role in these disorders .
	manualset3
262737	5	426227	7	NULL	NULL	NULL	NULL	cutaneous gene therapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the ready access to the skin compared with solid internal organs , the challenges of cutaneous gene therapy are legion and many technical issues need to be surmounted to enable gene replacement or modification of gene expression to have a useful role in these disorders .
	manualset3
262739	6	426227	7	NULL	NULL	NULL	NULL	 legion 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the ready access to the skin compared with solid internal organs , the challenges of cutaneous gene therapy are legion and many technical issues need to be surmounted to enable gene replacement or modification of gene expression to have a useful role in these disorders .
	manualset3
262740	7	426227	7	NULL	NULL	NULL	NULL	technical issues	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the ready access to the skin compared with solid internal organs , the challenges of cutaneous gene therapy are legion and many technical issues need to be surmounted to enable gene replacement or modification of gene expression to have a useful role in these disorders .
	manualset3
262741	8	426227	7	NULL	NULL	NULL	NULL	gene replacement 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the ready access to the skin compared with solid internal organs , the challenges of cutaneous gene therapy are legion and many technical issues need to be surmounted to enable gene replacement or modification of gene expression to have a useful role in these disorders .
	manualset3
262742	9	426227	7	NULL	NULL	NULL	NULL	modification	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the ready access to the skin compared with solid internal organs , the challenges of cutaneous gene therapy are legion and many technical issues need to be surmounted to enable gene replacement or modification of gene expression to have a useful role in these disorders .
	manualset3
262743	10	426227	7	NULL	NULL	NULL	NULL	gene expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the ready access to the skin compared with solid internal organs , the challenges of cutaneous gene therapy are legion and many technical issues need to be surmounted to enable gene replacement or modification of gene expression to have a useful role in these disorders .
	manualset3
262744	11	426227	7	NULL	NULL	NULL	NULL	disorders	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the ready access to the skin compared with solid internal organs , the challenges of cutaneous gene therapy are legion and many technical issues need to be surmounted to enable gene replacement or modification of gene expression to have a useful role in these disorders .
	manualset3
262745	1	426228	7	NULL	NULL	NULL	NULL	strong tumour-suppressing qualities	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the strong tumour-suppressing qualities of AC7700 , it does not produce an immediate reduction in tumor size .
	manualset3
262746	2	426228	7	NULL	NULL	NULL	NULL	AC7700 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the strong tumour-suppressing qualities of AC7700 , it does not produce an immediate reduction in tumor size .
	manualset3
262747	3	426228	7	NULL	NULL	NULL	NULL	 immediate reduction	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the strong tumour-suppressing qualities of AC7700 , it does not produce an immediate reduction in tumor size .
	manualset3
262748	4	426228	7	NULL	NULL	NULL	NULL	tumor size	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the strong tumour-suppressing qualities of AC7700 , it does not produce an immediate reduction in tumor size .
	manualset3
262749	1	426229	7	NULL	NULL	NULL	NULL	 presence 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the uncertainty as to the presence and biophysical properties of prions in plasma , prion removal studies have been conducted using brain homogenate or microsomes prepared from prion-infected rodent brains as model prions .
	manualset3
262750	2	426229	7	NULL	NULL	NULL	NULL	biophysical properties	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the uncertainty as to the presence and biophysical properties of prions in plasma , prion removal studies have been conducted using brain homogenate or microsomes prepared from prion-infected rodent brains as model prions .
	manualset3
262751	3	426229	7	NULL	NULL	NULL	NULL	prions	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the uncertainty as to the presence and biophysical properties of prions in plasma , prion removal studies have been conducted using brain homogenate or microsomes prepared from prion-infected rodent brains as model prions .
	manualset3
262752	4	426229	7	NULL	NULL	NULL	NULL	plasma	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the uncertainty as to the presence and biophysical properties of prions in plasma , prion removal studies have been conducted using brain homogenate or microsomes prepared from prion-infected rodent brains as model prions .
	manualset3
262753	5	426229	7	NULL	NULL	NULL	NULL	prion removal studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the uncertainty as to the presence and biophysical properties of prions in plasma , prion removal studies have been conducted using brain homogenate or microsomes prepared from prion-infected rodent brains as model prions .
	manualset3
262754	6	426229	7	NULL	NULL	NULL	NULL	brain homogenate 	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the uncertainty as to the presence and biophysical properties of prions in plasma , prion removal studies have been conducted using brain homogenate or microsomes prepared from prion-infected rodent brains as model prions .
	manualset3
262755	7	426229	7	NULL	NULL	NULL	NULL	 microsomes	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the uncertainty as to the presence and biophysical properties of prions in plasma , prion removal studies have been conducted using brain homogenate or microsomes prepared from prion-infected rodent brains as model prions .
	manualset3
262756	8	426229	7	NULL	NULL	NULL	NULL	prion-infected rodent brains	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the uncertainty as to the presence and biophysical properties of prions in plasma , prion removal studies have been conducted using brain homogenate or microsomes prepared from prion-infected rodent brains as model prions .
	manualset3
262757	9	426229	7	NULL	NULL	NULL	NULL	model prions	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the uncertainty as to the presence and biophysical properties of prions in plasma , prion removal studies have been conducted using brain homogenate or microsomes prepared from prion-infected rodent brains as model prions .
	manualset3
262758	1	426230	7	NULL	NULL	NULL	NULL	variation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the variation in materials and procedures employed by the three laboratories , repeatable and reproducible ` true ' ( 2 ) H isotope values ( ( 2 ) H ( hair , true ) ) were determined by each laboratory for each of the four stock samples of human scalp hair .
	manualset3
262759	2	426230	7	NULL	NULL	NULL	NULL	materials	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the variation in materials and procedures employed by the three laboratories , repeatable and reproducible ` true ' ( 2 ) H isotope values ( ( 2 ) H ( hair , true ) ) were determined by each laboratory for each of the four stock samples of human scalp hair .
	manualset3
262760	3	426230	7	NULL	NULL	NULL	NULL	procedures	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the variation in materials and procedures employed by the three laboratories , repeatable and reproducible ` true ' ( 2 ) H isotope values ( ( 2 ) H ( hair , true ) ) were determined by each laboratory for each of the four stock samples of human scalp hair .
	manualset3
262761	4	426230	7	NULL	NULL	NULL	NULL	three laboratories	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the variation in materials and procedures employed by the three laboratories , repeatable and reproducible ` true ' ( 2 ) H isotope values ( ( 2 ) H ( hair , true ) ) were determined by each laboratory for each of the four stock samples of human scalp hair .
	manualset3
262762	5	426230	7	NULL	NULL	NULL	NULL	 ` true ' ( 2 ) H isotope values ( ( 2 ) H ( hair , true ) )	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the variation in materials and procedures employed by the three laboratories , repeatable and reproducible ` true ' ( 2 ) H isotope values ( ( 2 ) H ( hair , true ) ) were determined by each laboratory for each of the four stock samples of human scalp hair .
	manualset3
262763	6	426230	7	NULL	NULL	NULL	NULL	 laboratory	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the variation in materials and procedures employed by the three laboratories , repeatable and reproducible ` true ' ( 2 ) H isotope values ( ( 2 ) H ( hair , true ) ) were determined by each laboratory for each of the four stock samples of human scalp hair .
	manualset3
262764	7	426230	7	NULL	NULL	NULL	NULL	four stock samples	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the variation in materials and procedures employed by the three laboratories , repeatable and reproducible ` true ' ( 2 ) H isotope values ( ( 2 ) H ( hair , true ) ) were determined by each laboratory for each of the four stock samples of human scalp hair .
	manualset3
262765	8	426230	7	NULL	NULL	NULL	NULL	human scalp hair	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite the variation in materials and procedures employed by the three laboratories , repeatable and reproducible ` true ' ( 2 ) H isotope values ( ( 2 ) H ( hair , true ) ) were determined by each laboratory for each of the four stock samples of human scalp hair .
	manualset3
262997	1	426231	7	NULL	NULL	NULL	NULL	research model	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite their importance as a research model , particularly in developmental toxicology investigations , there are few established standards for maintaining Xenopus spp .
	manualset3
262998	2	426231	7	NULL	NULL	NULL	NULL	developmental toxicology investigations 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite their importance as a research model , particularly in developmental toxicology investigations , there are few established standards for maintaining Xenopus spp .
	manualset3
262999	3	426231	7	NULL	NULL	NULL	NULL	 established standards	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite their importance as a research model , particularly in developmental toxicology investigations , there are few established standards for maintaining Xenopus spp .
	manualset3
263000	4	426231	7	NULL	NULL	NULL	NULL	Xenopus spp	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite their importance as a research model , particularly in developmental toxicology investigations , there are few established standards for maintaining Xenopus spp .
	manualset3
263004	1	426232	7	NULL	NULL	NULL	NULL	drastic modifications	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite these drastic modifications in PL fatty acid composition , the maximum velocity ( Vm ) of SR Ca2 + , Mg2 + - ATPase was not affected , which indicates that SR cardiac membrane adapts to changes in fatty acid composition to prevent important modifications of its functional properties .
	manualset3
263005	2	426232	7	NULL	NULL	NULL	NULL	PL fatty acid composition	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite these drastic modifications in PL fatty acid composition , the maximum velocity ( Vm ) of SR Ca2 + , Mg2 + - ATPase was not affected , which indicates that SR cardiac membrane adapts to changes in fatty acid composition to prevent important modifications of its functional properties .
	manualset3
263006	3	426232	7	NULL	NULL	NULL	NULL	 maximum velocity ( Vm )	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite these drastic modifications in PL fatty acid composition , the maximum velocity ( Vm ) of SR Ca2 + , Mg2 + - ATPase was not affected , which indicates that SR cardiac membrane adapts to changes in fatty acid composition to prevent important modifications of its functional properties .
	manualset3
263014	4	426232	7	NULL	NULL	NULL	NULL	SR 	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite these drastic modifications in PL fatty acid composition , the maximum velocity ( Vm ) of SR Ca2 + , Mg2 + - ATPase was not affected , which indicates that SR cardiac membrane adapts to changes in fatty acid composition to prevent important modifications of its functional properties .
	manualset3
263015	5	426232	7	NULL	NULL	NULL	NULL	Ca2 +	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite these drastic modifications in PL fatty acid composition , the maximum velocity ( Vm ) of SR Ca2 + , Mg2 + - ATPase was not affected , which indicates that SR cardiac membrane adapts to changes in fatty acid composition to prevent important modifications of its functional properties .
	manualset3
263018	6	426232	7	NULL	NULL	NULL	NULL	Mg2 + - ATPase	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite these drastic modifications in PL fatty acid composition , the maximum velocity ( Vm ) of SR Ca2 + , Mg2 + - ATPase was not affected , which indicates that SR cardiac membrane adapts to changes in fatty acid composition to prevent important modifications of its functional properties .
	manualset3
263021	7	426232	7	NULL	NULL	NULL	NULL	SR cardiac membrane 	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite these drastic modifications in PL fatty acid composition , the maximum velocity ( Vm ) of SR Ca2 + , Mg2 + - ATPase was not affected , which indicates that SR cardiac membrane adapts to changes in fatty acid composition to prevent important modifications of its functional properties .
	manualset3
263024	8	426232	7	NULL	NULL	NULL	NULL	fatty acid composition 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite these drastic modifications in PL fatty acid composition , the maximum velocity ( Vm ) of SR Ca2 + , Mg2 + - ATPase was not affected , which indicates that SR cardiac membrane adapts to changes in fatty acid composition to prevent important modifications of its functional properties .
	manualset3
263026	9	426232	7	NULL	NULL	NULL	NULL	important modifications	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite these drastic modifications in PL fatty acid composition , the maximum velocity ( Vm ) of SR Ca2 + , Mg2 + - ATPase was not affected , which indicates that SR cardiac membrane adapts to changes in fatty acid composition to prevent important modifications of its functional properties .
	manualset3
263030	10	426232	7	NULL	NULL	NULL	NULL	 functional properties	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite these drastic modifications in PL fatty acid composition , the maximum velocity ( Vm ) of SR Ca2 + , Mg2 + - ATPase was not affected , which indicates that SR cardiac membrane adapts to changes in fatty acid composition to prevent important modifications of its functional properties .
	manualset3
263041	1	426233	7	NULL	NULL	NULL	NULL	 ` homosexuality ' 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this , ` homosexuality ' continues to be treated as an unproblematic category in HIV/AIDS discourse , epidemiological studies of and HIV prevention strategies for MSM in widely different contexts being based on the North American/West European example of gay men .
	manualset3
263045	2	426233	7	NULL	NULL	NULL	NULL	unproblematic category	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this , ` homosexuality ' continues to be treated as an unproblematic category in HIV/AIDS discourse , epidemiological studies of and HIV prevention strategies for MSM in widely different contexts being based on the North American/West European example of gay men .
	manualset3
263048	3	426233	7	NULL	NULL	NULL	NULL	HIV/AIDS discourse	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this , ` homosexuality ' continues to be treated as an unproblematic category in HIV/AIDS discourse , epidemiological studies of and HIV prevention strategies for MSM in widely different contexts being based on the North American/West European example of gay men .
	manualset3
263049	4	426233	7	NULL	NULL	NULL	NULL	 epidemiological studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this , ` homosexuality ' continues to be treated as an unproblematic category in HIV/AIDS discourse , epidemiological studies of and HIV prevention strategies for MSM in widely different contexts being based on the North American/West European example of gay men .
	manualset3
263054	5	426233	7	NULL	NULL	NULL	NULL	HIV prevention strategies	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this , ` homosexuality ' continues to be treated as an unproblematic category in HIV/AIDS discourse , epidemiological studies of and HIV prevention strategies for MSM in widely different contexts being based on the North American/West European example of gay men .
	manualset3
263055	6	426233	7	NULL	NULL	NULL	NULL	MSM	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this , ` homosexuality ' continues to be treated as an unproblematic category in HIV/AIDS discourse , epidemiological studies of and HIV prevention strategies for MSM in widely different contexts being based on the North American/West European example of gay men .
	manualset3
263058	7	426233	7	NULL	NULL	NULL	NULL	different contexts	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this , ` homosexuality ' continues to be treated as an unproblematic category in HIV/AIDS discourse , epidemiological studies of and HIV prevention strategies for MSM in widely different contexts being based on the North American/West European example of gay men .
	manualset3
263059	8	426233	7	NULL	NULL	NULL	NULL	North American/West European example 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this , ` homosexuality ' continues to be treated as an unproblematic category in HIV/AIDS discourse , epidemiological studies of and HIV prevention strategies for MSM in widely different contexts being based on the North American/West European example of gay men .
	manualset3
263061	9	426233	7	NULL	NULL	NULL	NULL	gay men	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this , ` homosexuality ' continues to be treated as an unproblematic category in HIV/AIDS discourse , epidemiological studies of and HIV prevention strategies for MSM in widely different contexts being based on the North American/West European example of gay men .
	manualset3
263075	1	426234	7	NULL	NULL	NULL	NULL	level	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this level of DNA homology throughout the genome , both phages combined have 15 unique genes that do not occur in the other phage .
	manualset3
263078	2	426234	7	NULL	NULL	NULL	NULL	DNA homology	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this level of DNA homology throughout the genome , both phages combined have 15 unique genes that do not occur in the other phage .
	manualset3
263079	3	426234	7	NULL	NULL	NULL	NULL	genome	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this level of DNA homology throughout the genome , both phages combined have 15 unique genes that do not occur in the other phage .
	manualset3
263080	4	426234	7	NULL	NULL	NULL	NULL	phages	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this level of DNA homology throughout the genome , both phages combined have 15 unique genes that do not occur in the other phage .
	manualset3
263105	5	426234	7	NULL	NULL	NULL	NULL	15 unique genes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this level of DNA homology throughout the genome , both phages combined have 15 unique genes that do not occur in the other phage .
	manualset3
263106	6	426234	7	NULL	NULL	NULL	NULL	phage	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this level of DNA homology throughout the genome , both phages combined have 15 unique genes that do not occur in the other phage .
	manualset3
263118	1	426235	7	NULL	NULL	NULL	NULL	 limitation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this limitation , at least some of these molecules have been implicated in the control of differentiation and morphogenesis , two actions unpredicted from the cell biology of most of the growth factors .
	manualset3
263119	2	426235	7	NULL	NULL	NULL	NULL	 molecules	Molecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this limitation , at least some of these molecules have been implicated in the control of differentiation and morphogenesis , two actions unpredicted from the cell biology of most of the growth factors .
	manualset3
263122	3	426235	7	NULL	NULL	NULL	NULL	 control	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this limitation , at least some of these molecules have been implicated in the control of differentiation and morphogenesis , two actions unpredicted from the cell biology of most of the growth factors .
	manualset3
263124	4	426235	7	NULL	NULL	NULL	NULL	differentiation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this limitation , at least some of these molecules have been implicated in the control of differentiation and morphogenesis , two actions unpredicted from the cell biology of most of the growth factors .
	manualset3
263127	5	426235	7	NULL	NULL	NULL	NULL	morphogenesis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this limitation , at least some of these molecules have been implicated in the control of differentiation and morphogenesis , two actions unpredicted from the cell biology of most of the growth factors .
	manualset3
263130	6	426235	7	NULL	NULL	NULL	NULL	two actions	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this limitation , at least some of these molecules have been implicated in the control of differentiation and morphogenesis , two actions unpredicted from the cell biology of most of the growth factors .
	manualset3
263132	7	426235	7	NULL	NULL	NULL	NULL	cell biology	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this limitation , at least some of these molecules have been implicated in the control of differentiation and morphogenesis , two actions unpredicted from the cell biology of most of the growth factors .
	manualset3
263134	8	426235	7	NULL	NULL	NULL	NULL	growth factors	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this limitation , at least some of these molecules have been implicated in the control of differentiation and morphogenesis , two actions unpredicted from the cell biology of most of the growth factors .
	manualset3
263198	1	426236	7	NULL	NULL	NULL	NULL	 pretreatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this pretreatment , cold-restraint stress still induced ulcer formation , along with changes in gastric ir-TRH and ir-SOM concentrations and gastric pH. .
	manualset3
263200	2	426236	7	NULL	NULL	NULL	NULL	 cold-restraint stress	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this pretreatment , cold-restraint stress still induced ulcer formation , along with changes in gastric ir-TRH and ir-SOM concentrations and gastric pH. .
	manualset3
263203	3	426236	7	NULL	NULL	NULL	NULL	ulcer formation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this pretreatment , cold-restraint stress still induced ulcer formation , along with changes in gastric ir-TRH and ir-SOM concentrations and gastric pH. .
	manualset3
263205	4	426236	7	NULL	NULL	NULL	NULL	changes	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this pretreatment , cold-restraint stress still induced ulcer formation , along with changes in gastric ir-TRH and ir-SOM concentrations and gastric pH. .
	manualset3
263208	5	426236	7	NULL	NULL	NULL	NULL	gastric ir-TRH concentrations	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this pretreatment , cold-restraint stress still induced ulcer formation , along with changes in gastric ir-TRH and ir-SOM concentrations and gastric pH. .
	manualset3
263211	6	426236	7	NULL	NULL	NULL	NULL	 ir-SOM concentrations 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this pretreatment , cold-restraint stress still induced ulcer formation , along with changes in gastric ir-TRH and ir-SOM concentrations and gastric pH. .
	manualset3
263214	7	426236	7	NULL	NULL	NULL	NULL	gastric pH	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite this pretreatment , cold-restraint stress still induced ulcer formation , along with changes in gastric ir-TRH and ir-SOM concentrations and gastric pH. .
	manualset3
263225	1	426237	7	NULL	NULL	NULL	NULL	 treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite treatment with antifungal therapy , she required a laparotomy owing to severe hemorrhage caused by mucormycosal invasion of her iliac artery .
	manualset3
263226	2	426237	7	NULL	NULL	NULL	NULL	antifungal therapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite treatment with antifungal therapy , she required a laparotomy owing to severe hemorrhage caused by mucormycosal invasion of her iliac artery .
	manualset3
263227	3	426237	7	NULL	NULL	NULL	NULL	laparotomy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite treatment with antifungal therapy , she required a laparotomy owing to severe hemorrhage caused by mucormycosal invasion of her iliac artery .
	manualset3
263228	4	426237	7	NULL	NULL	NULL	NULL	severe hemorrhage	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite treatment with antifungal therapy , she required a laparotomy owing to severe hemorrhage caused by mucormycosal invasion of her iliac artery .
	manualset3
263229	5	426237	7	NULL	NULL	NULL	NULL	mucormycosal invasion	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite treatment with antifungal therapy , she required a laparotomy owing to severe hemorrhage caused by mucormycosal invasion of her iliac artery .
	manualset3
263230	6	426237	7	NULL	NULL	NULL	NULL	 iliac artery 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Despite treatment with antifungal therapy , she required a laparotomy owing to severe hemorrhage caused by mucormycosal invasion of her iliac artery .
	manualset3
263231	1	426238	7	NULL	NULL	NULL	NULL	Destruction	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Destruction of pancreatic beta cells has been implicted in the progression to hyperglycemia in type 1 diabetes .
	manualset3
263232	2	426238	7	NULL	NULL	NULL	NULL	pancreatic beta cells 	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Destruction of pancreatic beta cells has been implicted in the progression to hyperglycemia in type 1 diabetes .
	manualset3
263233	3	426238	7	NULL	NULL	NULL	NULL	progression	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Destruction of pancreatic beta cells has been implicted in the progression to hyperglycemia in type 1 diabetes .
	manualset3
263234	4	426238	7	NULL	NULL	NULL	NULL	 hyperglycemia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Destruction of pancreatic beta cells has been implicted in the progression to hyperglycemia in type 1 diabetes .
	manualset3
263235	5	426238	7	NULL	NULL	NULL	NULL	type 1 diabetes	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Destruction of pancreatic beta cells has been implicted in the progression to hyperglycemia in type 1 diabetes .
	manualset3
263236	1	426239	7	NULL	NULL	NULL	NULL	Detailed analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detailed analysis and endoscopy were used to differentiate the symptoms that were related to laryngomalacia from those that were caused by other conditions , including mixed-breathing , swallowing , and sucking difficulties .
	manualset3
263237	2	426239	7	NULL	NULL	NULL	NULL	endoscopy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detailed analysis and endoscopy were used to differentiate the symptoms that were related to laryngomalacia from those that were caused by other conditions , including mixed-breathing , swallowing , and sucking difficulties .
	manualset3
263238	3	426239	7	NULL	NULL	NULL	NULL	symptoms	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detailed analysis and endoscopy were used to differentiate the symptoms that were related to laryngomalacia from those that were caused by other conditions , including mixed-breathing , swallowing , and sucking difficulties .
	manualset3
263239	4	426239	7	NULL	NULL	NULL	NULL	 laryngomalacia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detailed analysis and endoscopy were used to differentiate the symptoms that were related to laryngomalacia from those that were caused by other conditions , including mixed-breathing , swallowing , and sucking difficulties .
	manualset3
263240	5	426239	7	NULL	NULL	NULL	NULL	conditions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detailed analysis and endoscopy were used to differentiate the symptoms that were related to laryngomalacia from those that were caused by other conditions , including mixed-breathing , swallowing , and sucking difficulties .
	manualset3
263241	6	426239	7	NULL	NULL	NULL	NULL	mixed-breathing	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detailed analysis and endoscopy were used to differentiate the symptoms that were related to laryngomalacia from those that were caused by other conditions , including mixed-breathing , swallowing , and sucking difficulties .
	manualset3
263242	7	426239	7	NULL	NULL	NULL	NULL	swallowing	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detailed analysis and endoscopy were used to differentiate the symptoms that were related to laryngomalacia from those that were caused by other conditions , including mixed-breathing , swallowing , and sucking difficulties .
	manualset3
263243	8	426239	7	NULL	NULL	NULL	NULL	sucking difficulties	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detailed analysis and endoscopy were used to differentiate the symptoms that were related to laryngomalacia from those that were caused by other conditions , including mixed-breathing , swallowing , and sucking difficulties .
	manualset3
263244	1	426240	7	NULL	NULL	NULL	NULL	hemodynamic course	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detailed hemodynamic course during prolonged ( less than 12 h ) septic shock was studied in 23 patients , of whom 12 ultimately died from sepsis .
	manualset3
263245	2	426240	7	NULL	NULL	NULL	NULL	prolonged septic shock	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detailed hemodynamic course during prolonged ( less than 12 h ) septic shock was studied in 23 patients , of whom 12 ultimately died from sepsis .
	manualset3
263246	3	426240	7	NULL	NULL	NULL	NULL	12 h 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detailed hemodynamic course during prolonged ( less than 12 h ) septic shock was studied in 23 patients , of whom 12 ultimately died from sepsis .
	manualset3
263247	4	426240	7	NULL	NULL	NULL	NULL	 23 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detailed hemodynamic course during prolonged ( less than 12 h ) septic shock was studied in 23 patients , of whom 12 ultimately died from sepsis .
	manualset3
263248	5	426240	7	NULL	NULL	NULL	NULL	12 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detailed hemodynamic course during prolonged ( less than 12 h ) septic shock was studied in 23 patients , of whom 12 ultimately died from sepsis .
	manualset3
263249	6	426240	7	NULL	NULL	NULL	NULL	sepsis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detailed hemodynamic course during prolonged ( less than 12 h ) septic shock was studied in 23 patients , of whom 12 ultimately died from sepsis .
	manualset3
263250	1	426241	7	NULL	NULL	NULL	NULL	investigation 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detailed investigation by urethroscopy , biopsy , CT imaging and ultrasonography revealed epidermoid carcinoma of the urethra .
	manualset3
263251	2	426241	7	NULL	NULL	NULL	NULL	urethroscopy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detailed investigation by urethroscopy , biopsy , CT imaging and ultrasonography revealed epidermoid carcinoma of the urethra .
	manualset3
263252	3	426241	7	NULL	NULL	NULL	NULL	biopsy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detailed investigation by urethroscopy , biopsy , CT imaging and ultrasonography revealed epidermoid carcinoma of the urethra .
	manualset3
263253	4	426241	7	NULL	NULL	NULL	NULL	CT imaging	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detailed investigation by urethroscopy , biopsy , CT imaging and ultrasonography revealed epidermoid carcinoma of the urethra .
	manualset3
263254	5	426241	7	NULL	NULL	NULL	NULL	ultrasonography	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detailed investigation by urethroscopy , biopsy , CT imaging and ultrasonography revealed epidermoid carcinoma of the urethra .
	manualset3
263255	6	426241	7	NULL	NULL	NULL	NULL	epidermoid carcinoma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detailed investigation by urethroscopy , biopsy , CT imaging and ultrasonography revealed epidermoid carcinoma of the urethra .
	manualset3
263256	7	426241	7	NULL	NULL	NULL	NULL	urethra	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detailed investigation by urethroscopy , biopsy , CT imaging and ultrasonography revealed epidermoid carcinoma of the urethra .
	manualset3
263257	1	426242	7	NULL	NULL	NULL	NULL	 kinetic  characterisation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detailed kinetic and physiological characterisation of eight mannitol-producing lactic acid bacteria , Leuconostoc citreum ATCC 49370 , L. mesenteroides subsp .
	manualset3
263258	2	426242	7	NULL	NULL	NULL	NULL	 physiological characterisation 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detailed kinetic and physiological characterisation of eight mannitol-producing lactic acid bacteria , Leuconostoc citreum ATCC 49370 , L. mesenteroides subsp .
	manualset3
263259	3	426242	7	NULL	NULL	NULL	NULL	 eight	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detailed kinetic and physiological characterisation of eight mannitol-producing lactic acid bacteria , Leuconostoc citreum ATCC 49370 , L. mesenteroides subsp .
	manualset3
263260	4	426242	7	NULL	NULL	NULL	NULL	mannitol-producing lactic acid bacteria	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detailed kinetic and physiological characterisation of eight mannitol-producing lactic acid bacteria , Leuconostoc citreum ATCC 49370 , L. mesenteroides subsp .
	manualset3
263261	5	426242	7	NULL	NULL	NULL	NULL	Leuconostoc citreum ATCC 49370	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detailed kinetic and physiological characterisation of eight mannitol-producing lactic acid bacteria , Leuconostoc citreum ATCC 49370 , L. mesenteroides subsp .
	manualset3
263262	6	426242	7	NULL	NULL	NULL	NULL	L. mesenteroides subsp	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detailed kinetic and physiological characterisation of eight mannitol-producing lactic acid bacteria , Leuconostoc citreum ATCC 49370 , L. mesenteroides subsp .
	manualset3
263263	1	426243	7	NULL	NULL	NULL	NULL	Detection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection and analysis of hair .
	manualset3
263264	2	426243	7	NULL	NULL	NULL	NULL	analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection and analysis of hair .
	manualset3
263265	3	426243	7	NULL	NULL	NULL	NULL	hair 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection and analysis of hair .
	manualset3
263266	1	426244	7	NULL	NULL	NULL	NULL	Detection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection and assessment of coronary artery anomalies by three-dimensional magnetic resonance coronary angiography .
	manualset3
263267	2	426244	7	NULL	NULL	NULL	NULL	assessment 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection and assessment of coronary artery anomalies by three-dimensional magnetic resonance coronary angiography .
	manualset3
263268	3	426244	7	NULL	NULL	NULL	NULL	coronary artery anomalies	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection and assessment of coronary artery anomalies by three-dimensional magnetic resonance coronary angiography .
	manualset3
263269	4	426244	7	NULL	NULL	NULL	NULL	three-dimensional magnetic resonance coronary angiography	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection and assessment of coronary artery anomalies by three-dimensional magnetic resonance coronary angiography .
	manualset3
263270	1	426245	7	NULL	NULL	NULL	NULL	Detection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection and quantification of phosphotyrosine in proteins .
	manualset3
263271	2	426245	7	NULL	NULL	NULL	NULL	 quantification	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection and quantification of phosphotyrosine in proteins .
	manualset3
263272	3	426245	7	NULL	NULL	NULL	NULL	phosphotyrosine	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection and quantification of phosphotyrosine in proteins .
	manualset3
263273	4	426245	7	NULL	NULL	NULL	NULL	proteins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection and quantification of phosphotyrosine in proteins .
	manualset3
263274	1	426246	7	NULL	NULL	NULL	NULL	Detection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection and quantitation of infectious human adenoviruses and JC polyomaviruses in water by immunofluorescence assay .
	manualset3
263275	2	426246	7	NULL	NULL	NULL	NULL	 quantitation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection and quantitation of infectious human adenoviruses and JC polyomaviruses in water by immunofluorescence assay .
	manualset3
263276	3	426246	7	NULL	NULL	NULL	NULL	 infectious human adenoviruses 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection and quantitation of infectious human adenoviruses and JC polyomaviruses in water by immunofluorescence assay .
	manualset3
263277	4	426246	7	NULL	NULL	NULL	NULL	JC polyomaviruses	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection and quantitation of infectious human adenoviruses and JC polyomaviruses in water by immunofluorescence assay .
	manualset3
263278	5	426246	7	NULL	NULL	NULL	NULL	water	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection and quantitation of infectious human adenoviruses and JC polyomaviruses in water by immunofluorescence assay .
	manualset3
263279	6	426246	7	NULL	NULL	NULL	NULL	immunofluorescence assay 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection and quantitation of infectious human adenoviruses and JC polyomaviruses in water by immunofluorescence assay .
	manualset3
263280	1	426247	7	NULL	NULL	NULL	NULL	Detection limits	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection limits were 0.074 / 0.119 microg/ml and 0.072 / 0.116 microg/ml for CN/DOM and CN/NIC , respectively .
	manualset3
263281	2	426247	7	NULL	NULL	NULL	NULL	 0.074 / 0.119 microg/ml	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection limits were 0.074 / 0.119 microg/ml and 0.072 / 0.116 microg/ml for CN/DOM and CN/NIC , respectively .
	manualset3
263282	3	426247	7	NULL	NULL	NULL	NULL	0.072 / 0.116 microg/ml 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection limits were 0.074 / 0.119 microg/ml and 0.072 / 0.116 microg/ml for CN/DOM and CN/NIC , respectively .
	manualset3
263283	4	426247	7	NULL	NULL	NULL	NULL	 CN/DOM	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection limits were 0.074 / 0.119 microg/ml and 0.072 / 0.116 microg/ml for CN/DOM and CN/NIC , respectively .
	manualset3
263284	5	426247	7	NULL	NULL	NULL	NULL	CN/NIC	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection limits were 0.074 / 0.119 microg/ml and 0.072 / 0.116 microg/ml for CN/DOM and CN/NIC , respectively .
	manualset3
263285	1	426248	7	NULL	NULL	NULL	NULL	Detection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of CMV DNA by PCR was a more rapid and sensitive technique than conventional culture .
	manualset3
263286	2	426248	7	NULL	NULL	NULL	NULL	CMV DNA	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of CMV DNA by PCR was a more rapid and sensitive technique than conventional culture .
	manualset3
263287	3	426248	7	NULL	NULL	NULL	NULL	PCR	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of CMV DNA by PCR was a more rapid and sensitive technique than conventional culture .
	manualset3
263288	4	426248	7	NULL	NULL	NULL	NULL	 sensitive technique	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of CMV DNA by PCR was a more rapid and sensitive technique than conventional culture .
	manualset3
263289	5	426248	7	NULL	NULL	NULL	NULL	culture	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of CMV DNA by PCR was a more rapid and sensitive technique than conventional culture .
	manualset3
263290	1	426249	7	NULL	NULL	NULL	NULL	Detection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of Chlamydophila psittaci by using SYBR green real-time PCR .
	manualset3
263291	2	426249	7	NULL	NULL	NULL	NULL	Chlamydophila psittaci	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of Chlamydophila psittaci by using SYBR green real-time PCR .
	manualset3
263292	3	426249	7	NULL	NULL	NULL	NULL	SYBR green real-time PCR	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of Chlamydophila psittaci by using SYBR green real-time PCR .
	manualset3
263293	1	426250	7	NULL	NULL	NULL	NULL	Detection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of TTV was conducted by nested PCR and real-time PCR in the sera of 94 patients with IIM , 95 RA patients .
	manualset3
263294	2	426250	7	NULL	NULL	NULL	NULL	TTV	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of TTV was conducted by nested PCR and real-time PCR in the sera of 94 patients with IIM , 95 RA patients .
	manualset3
263295	3	426250	7	NULL	NULL	NULL	NULL	nested PCR	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of TTV was conducted by nested PCR and real-time PCR in the sera of 94 patients with IIM , 95 RA patients .
	manualset3
263296	4	426250	7	NULL	NULL	NULL	NULL	real-time PCR	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of TTV was conducted by nested PCR and real-time PCR in the sera of 94 patients with IIM , 95 RA patients .
	manualset3
263297	5	426250	7	NULL	NULL	NULL	NULL	sera	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of TTV was conducted by nested PCR and real-time PCR in the sera of 94 patients with IIM , 95 RA patients .
	manualset3
263298	6	426250	7	NULL	NULL	NULL	NULL	94 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of TTV was conducted by nested PCR and real-time PCR in the sera of 94 patients with IIM , 95 RA patients .
	manualset3
263299	7	426250	7	NULL	NULL	NULL	NULL	 IIM	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of TTV was conducted by nested PCR and real-time PCR in the sera of 94 patients with IIM , 95 RA patients .
	manualset3
263300	8	426250	7	NULL	NULL	NULL	NULL	 95 RA patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of TTV was conducted by nested PCR and real-time PCR in the sera of 94 patients with IIM , 95 RA patients .
	manualset3
263301	1	426251	7	NULL	NULL	NULL	NULL	Detection 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of a beta-gal activity in SPC-SL 52 cells following several subcultures post-transfection suggests that Jlac Z recombinant genome could be maintained in an integrative or episomal state .
	manualset3
263302	2	426251	7	NULL	NULL	NULL	NULL	beta-gal activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of a beta-gal activity in SPC-SL 52 cells following several subcultures post-transfection suggests that Jlac Z recombinant genome could be maintained in an integrative or episomal state .
	manualset3
263303	3	426251	7	NULL	NULL	NULL	NULL	SPC-SL 52 cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of a beta-gal activity in SPC-SL 52 cells following several subcultures post-transfection suggests that Jlac Z recombinant genome could be maintained in an integrative or episomal state .
	manualset3
263304	4	426251	7	NULL	NULL	NULL	NULL	subcultures post-transfection	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of a beta-gal activity in SPC-SL 52 cells following several subcultures post-transfection suggests that Jlac Z recombinant genome could be maintained in an integrative or episomal state .
	manualset3
263305	5	426251	7	NULL	NULL	NULL	NULL	Jlac Z recombinant genome	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of a beta-gal activity in SPC-SL 52 cells following several subcultures post-transfection suggests that Jlac Z recombinant genome could be maintained in an integrative or episomal state .
	manualset3
263306	6	426251	7	NULL	NULL	NULL	NULL	integrative state	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of a beta-gal activity in SPC-SL 52 cells following several subcultures post-transfection suggests that Jlac Z recombinant genome could be maintained in an integrative or episomal state .
	manualset3
263307	7	426251	7	NULL	NULL	NULL	NULL	episomal state .	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of a beta-gal activity in SPC-SL 52 cells following several subcultures post-transfection suggests that Jlac Z recombinant genome could be maintained in an integrative or episomal state .
	manualset3
263308	1	426252	7	NULL	NULL	NULL	NULL	Detection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of brachytherapy seeds using 3D ultrasound .
	manualset3
263309	2	426252	7	NULL	NULL	NULL	NULL	 brachytherapy seeds	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of brachytherapy seeds using 3D ultrasound .
	manualset3
263310	3	426252	7	NULL	NULL	NULL	NULL	3D ultrasound 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of brachytherapy seeds using 3D ultrasound .
	manualset3
263311	1	426253	7	NULL	NULL	NULL	NULL	Detection 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of differentiation in acute promyelocytic leukemia .
	manualset3
263312	2	426253	7	NULL	NULL	NULL	NULL	differentiation 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of differentiation in acute promyelocytic leukemia .
	manualset3
263313	3	426253	7	NULL	NULL	NULL	NULL	acute promyelocytic leukemia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of differentiation in acute promyelocytic leukemia .
	manualset3
263314	1	426254	7	NULL	NULL	NULL	NULL	New views	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( New views on the radiotherapy of cervical cancer ) .
	manualset3
263315	2	426254	7	NULL	NULL	NULL	NULL	 radiotherapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( New views on the radiotherapy of cervical cancer ) .
	manualset3
263316	3	426254	7	NULL	NULL	NULL	NULL	 cervical cancer	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( New views on the radiotherapy of cervical cancer ) .
	manualset3
263317	1	426255	7	NULL	NULL	NULL	NULL	Detection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of fexofenadine and IS was achieved by LC-MS/MS in positive ion mode using 502.1 -- ) 466.2 and 446.0 -- ) 321.1 transitions , respectively .
	manualset3
263318	2	426255	7	NULL	NULL	NULL	NULL	fexofenadine	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of fexofenadine and IS was achieved by LC-MS/MS in positive ion mode using 502.1 -- ) 466.2 and 446.0 -- ) 321.1 transitions , respectively .
	manualset3
263319	3	426255	7	NULL	NULL	NULL	NULL	IS	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of fexofenadine and IS was achieved by LC-MS/MS in positive ion mode using 502.1 -- ) 466.2 and 446.0 -- ) 321.1 transitions , respectively .
	manualset3
263320	4	426255	7	NULL	NULL	NULL	NULL	LC-MS/MS	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of fexofenadine and IS was achieved by LC-MS/MS in positive ion mode using 502.1 -- ) 466.2 and 446.0 -- ) 321.1 transitions , respectively .
	manualset3
263321	5	426255	7	NULL	NULL	NULL	NULL	positive ion mode	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of fexofenadine and IS was achieved by LC-MS/MS in positive ion mode using 502.1 -- ) 466.2 and 446.0 -- ) 321.1 transitions , respectively .
	manualset3
263322	6	426255	7	NULL	NULL	NULL	NULL	502.1 -- ) transitions	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of fexofenadine and IS was achieved by LC-MS/MS in positive ion mode using 502.1 -- ) 466.2 and 446.0 -- ) 321.1 transitions , respectively .
	manualset3
263323	7	426255	7	NULL	NULL	NULL	NULL	466.2 transitions	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of fexofenadine and IS was achieved by LC-MS/MS in positive ion mode using 502.1 -- ) 466.2 and 446.0 -- ) 321.1 transitions , respectively .
	manualset3
263324	8	426255	7	NULL	NULL	NULL	NULL	 446.0 -- ) transitions	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of fexofenadine and IS was achieved by LC-MS/MS in positive ion mode using 502.1 -- ) 466.2 and 446.0 -- ) 321.1 transitions , respectively .
	manualset3
263325	9	426255	7	NULL	NULL	NULL	NULL	321.1 transitions	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of fexofenadine and IS was achieved by LC-MS/MS in positive ion mode using 502.1 -- ) 466.2 and 446.0 -- ) 321.1 transitions , respectively .
	manualset3
263326	1	426256	7	NULL	NULL	NULL	NULL	Detection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of genetically modified microorganisms in soil using the most-probable-number method with multiplex PCR and DNA dot blot .
	manualset3
263327	2	426256	7	NULL	NULL	NULL	NULL	genetically modified microorganisms	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of genetically modified microorganisms in soil using the most-probable-number method with multiplex PCR and DNA dot blot .
	manualset3
263328	3	426256	7	NULL	NULL	NULL	NULL	soil 	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of genetically modified microorganisms in soil using the most-probable-number method with multiplex PCR and DNA dot blot .
	manualset3
263329	4	426256	7	NULL	NULL	NULL	NULL	most-probable-number method	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of genetically modified microorganisms in soil using the most-probable-number method with multiplex PCR and DNA dot blot .
	manualset3
263330	5	426256	7	NULL	NULL	NULL	NULL	multiplex PCR	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of genetically modified microorganisms in soil using the most-probable-number method with multiplex PCR and DNA dot blot .
	manualset3
263331	6	426256	7	NULL	NULL	NULL	NULL	DNA dot blot	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of genetically modified microorganisms in soil using the most-probable-number method with multiplex PCR and DNA dot blot .
	manualset3
263332	1	426257	7	NULL	NULL	NULL	NULL	Detection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of genotypic virulence marker ( 162-kb ) in the CSF 90356 isolate by PFGE emphasizes the high risk of invasive infection by some GBS-III strains .
	manualset3
263333	2	426257	7	NULL	NULL	NULL	NULL	genotypic virulence marker ( 162-kb )	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of genotypic virulence marker ( 162-kb ) in the CSF 90356 isolate by PFGE emphasizes the high risk of invasive infection by some GBS-III strains .
	manualset3
263334	3	426257	7	NULL	NULL	NULL	NULL	CSF 90356 isolate	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of genotypic virulence marker ( 162-kb ) in the CSF 90356 isolate by PFGE emphasizes the high risk of invasive infection by some GBS-III strains .
	manualset3
263335	4	426257	7	NULL	NULL	NULL	NULL	 PFGE	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of genotypic virulence marker ( 162-kb ) in the CSF 90356 isolate by PFGE emphasizes the high risk of invasive infection by some GBS-III strains .
	manualset3
263336	5	426257	7	NULL	NULL	NULL	NULL	high risk	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of genotypic virulence marker ( 162-kb ) in the CSF 90356 isolate by PFGE emphasizes the high risk of invasive infection by some GBS-III strains .
	manualset3
263337	6	426257	7	NULL	NULL	NULL	NULL	invasive infection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of genotypic virulence marker ( 162-kb ) in the CSF 90356 isolate by PFGE emphasizes the high risk of invasive infection by some GBS-III strains .
	manualset3
263338	7	426257	7	NULL	NULL	NULL	NULL	GBS-III strains 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of genotypic virulence marker ( 162-kb ) in the CSF 90356 isolate by PFGE emphasizes the high risk of invasive infection by some GBS-III strains .
	manualset3
263339	1	426258	7	NULL	NULL	NULL	NULL	Detection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of hepatic phenylalanine 4-hydroxylase in classical phenylketonuria .
	manualset3
263340	2	426258	7	NULL	NULL	NULL	NULL	hepatic phenylalanine 4-hydroxylase	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of hepatic phenylalanine 4-hydroxylase in classical phenylketonuria .
	manualset3
263341	3	426258	7	NULL	NULL	NULL	NULL	classical phenylketonuria	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of hepatic phenylalanine 4-hydroxylase in classical phenylketonuria .
	manualset3
263342	1	426259	7	NULL	NULL	NULL	NULL	Detection 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of high-temperature water vapor at 940 nm with vertical-cavity surface-emitting lasers .
	manualset3
263343	2	426259	7	NULL	NULL	NULL	NULL	high-temperature water vapor 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of high-temperature water vapor at 940 nm with vertical-cavity surface-emitting lasers .
	manualset3
263344	3	426259	7	NULL	NULL	NULL	NULL	940 nm	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of high-temperature water vapor at 940 nm with vertical-cavity surface-emitting lasers .
	manualset3
263345	4	426259	7	NULL	NULL	NULL	NULL	vertical-cavity surface-emitting lasers	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of high-temperature water vapor at 940 nm with vertical-cavity surface-emitting lasers .
	manualset3
263346	1	426260	7	NULL	NULL	NULL	NULL	Detection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of loss of heterozygosity in tumor DNA samples by PCR .
	manualset3
263347	2	426260	7	NULL	NULL	NULL	NULL	 loss of heterozygosity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of loss of heterozygosity in tumor DNA samples by PCR .
	manualset3
263348	3	426260	7	NULL	NULL	NULL	NULL	 tumor DNA samples	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of loss of heterozygosity in tumor DNA samples by PCR .
	manualset3
263349	4	426260	7	NULL	NULL	NULL	NULL	PCR	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of loss of heterozygosity in tumor DNA samples by PCR .
	manualset3
263350	1	426261	7	NULL	NULL	NULL	NULL	Detection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of measles virus genome in blood leucocytes of patients with certain autoimmune diseases .
	manualset3
263351	2	426261	7	NULL	NULL	NULL	NULL	measles virus genome	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of measles virus genome in blood leucocytes of patients with certain autoimmune diseases .
	manualset3
263352	3	426261	7	NULL	NULL	NULL	NULL	blood leucocytes	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of measles virus genome in blood leucocytes of patients with certain autoimmune diseases .
	manualset3
263353	4	426261	7	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of measles virus genome in blood leucocytes of patients with certain autoimmune diseases .
	manualset3
263354	5	426261	7	NULL	NULL	NULL	NULL	autoimmune diseases	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of measles virus genome in blood leucocytes of patients with certain autoimmune diseases .
	manualset3
263702	1	426262	7	NULL	NULL	NULL	NULL	Detection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of mitochondrial DNA from domestic cattle in bison on Santa Catalina Island .
	manualset3
263703	2	426262	7	NULL	NULL	NULL	NULL	mitochondrial DNA	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of mitochondrial DNA from domestic cattle in bison on Santa Catalina Island .
	manualset3
263704	3	426262	7	NULL	NULL	NULL	NULL	domestic cattle	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of mitochondrial DNA from domestic cattle in bison on Santa Catalina Island .
	manualset3
263705	4	426262	7	NULL	NULL	NULL	NULL	bison	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of mitochondrial DNA from domestic cattle in bison on Santa Catalina Island .
	manualset3
263707	5	426262	7	NULL	NULL	NULL	NULL	Santa Catalina Island 	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of mitochondrial DNA from domestic cattle in bison on Santa Catalina Island .
	manualset3
263710	1	426263	7	NULL	NULL	NULL	NULL	Detection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of telomerase activity in exfoliated cells in urine from patients with bladder cancer .
	manualset3
263711	2	426263	7	NULL	NULL	NULL	NULL	telomerase activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of telomerase activity in exfoliated cells in urine from patients with bladder cancer .
	manualset3
263713	3	426263	7	NULL	NULL	NULL	NULL	exfoliated cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of telomerase activity in exfoliated cells in urine from patients with bladder cancer .
	manualset3
263714	4	426263	7	NULL	NULL	NULL	NULL	urine	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of telomerase activity in exfoliated cells in urine from patients with bladder cancer .
	manualset3
263715	5	426263	7	NULL	NULL	NULL	NULL	patients 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of telomerase activity in exfoliated cells in urine from patients with bladder cancer .
	manualset3
263716	6	426263	7	NULL	NULL	NULL	NULL	bladder cancer	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Detection of telomerase activity in exfoliated cells in urine from patients with bladder cancer .
	manualset3
263718	1	426264	7	NULL	NULL	NULL	NULL	Nine cases	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Nine cases of spontaneous hemopneumothorax with massive bleeding ) .
	manualset3
263719	2	426264	7	NULL	NULL	NULL	NULL	spontaneous hemopneumothorax	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Nine cases of spontaneous hemopneumothorax with massive bleeding ) .
	manualset3
263720	3	426264	7	NULL	NULL	NULL	NULL	massive bleeding	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Nine cases of spontaneous hemopneumothorax with massive bleeding ) .
	manualset3
263721	1	426265	7	NULL	NULL	NULL	NULL	Determinants	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determinants of high-sensitivity troponin T among patients with a noncardiac cause of chest pain .
	manualset3
263722	2	426265	7	NULL	NULL	NULL	NULL	high-sensitivity troponin T	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determinants of high-sensitivity troponin T among patients with a noncardiac cause of chest pain .
	manualset3
263724	3	426265	7	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determinants of high-sensitivity troponin T among patients with a noncardiac cause of chest pain .
	manualset3
263726	4	426265	7	NULL	NULL	NULL	NULL	noncardiac cause	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determinants of high-sensitivity troponin T among patients with a noncardiac cause of chest pain .
	manualset3
263727	5	426265	7	NULL	NULL	NULL	NULL	chest pain	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determinants of high-sensitivity troponin T among patients with a noncardiac cause of chest pain .
	manualset3
263729	1	426266	7	NULL	NULL	NULL	NULL	Determinants	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determinants of weaning and survival among patients with COPD who require mechanical ventilation for acute respiratory failure .
	manualset3
263731	2	426266	7	NULL	NULL	NULL	NULL	weaning	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determinants of weaning and survival among patients with COPD who require mechanical ventilation for acute respiratory failure .
	manualset3
263733	3	426266	7	NULL	NULL	NULL	NULL	survival 	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determinants of weaning and survival among patients with COPD who require mechanical ventilation for acute respiratory failure .
	manualset3
263735	4	426266	7	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determinants of weaning and survival among patients with COPD who require mechanical ventilation for acute respiratory failure .
	manualset3
263737	5	426266	7	NULL	NULL	NULL	NULL	COPD	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determinants of weaning and survival among patients with COPD who require mechanical ventilation for acute respiratory failure .
	manualset3
263741	6	426266	7	NULL	NULL	NULL	NULL	mechanical ventilation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determinants of weaning and survival among patients with COPD who require mechanical ventilation for acute respiratory failure .
	manualset3
263743	7	426266	7	NULL	NULL	NULL	NULL	acute respiratory failure	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determinants of weaning and survival among patients with COPD who require mechanical ventilation for acute respiratory failure .
	manualset3
263745	1	426267	7	NULL	NULL	NULL	NULL	Determination	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of NEFA levels in arterial and coronary sinus blood in patients with AMI and their temporal dynamics may be helpful for evaluation of the degree of the disease severity and can also be of prognostic value .
	manualset3
263747	2	426267	7	NULL	NULL	NULL	NULL	NEFA levels	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of NEFA levels in arterial and coronary sinus blood in patients with AMI and their temporal dynamics may be helpful for evaluation of the degree of the disease severity and can also be of prognostic value .
	manualset3
263755	3	426267	7	NULL	NULL	NULL	NULL	arterial  sinus blood	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of NEFA levels in arterial and coronary sinus blood in patients with AMI and their temporal dynamics may be helpful for evaluation of the degree of the disease severity and can also be of prognostic value .
	manualset3
263760	4	426267	7	NULL	NULL	NULL	NULL	coronary sinus blood	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of NEFA levels in arterial and coronary sinus blood in patients with AMI and their temporal dynamics may be helpful for evaluation of the degree of the disease severity and can also be of prognostic value .
	manualset3
263763	5	426267	7	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of NEFA levels in arterial and coronary sinus blood in patients with AMI and their temporal dynamics may be helpful for evaluation of the degree of the disease severity and can also be of prognostic value .
	manualset3
263765	6	426267	7	NULL	NULL	NULL	NULL	AMI 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of NEFA levels in arterial and coronary sinus blood in patients with AMI and their temporal dynamics may be helpful for evaluation of the degree of the disease severity and can also be of prognostic value .
	manualset3
263766	7	426267	7	NULL	NULL	NULL	NULL	temporal dynamics	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of NEFA levels in arterial and coronary sinus blood in patients with AMI and their temporal dynamics may be helpful for evaluation of the degree of the disease severity and can also be of prognostic value .
	manualset3
263768	8	426267	7	NULL	NULL	NULL	NULL	evaluation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of NEFA levels in arterial and coronary sinus blood in patients with AMI and their temporal dynamics may be helpful for evaluation of the degree of the disease severity and can also be of prognostic value .
	manualset3
263770	9	426267	7	NULL	NULL	NULL	NULL	degree	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of NEFA levels in arterial and coronary sinus blood in patients with AMI and their temporal dynamics may be helpful for evaluation of the degree of the disease severity and can also be of prognostic value .
	manualset3
263771	10	426267	7	NULL	NULL	NULL	NULL	disease severity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of NEFA levels in arterial and coronary sinus blood in patients with AMI and their temporal dynamics may be helpful for evaluation of the degree of the disease severity and can also be of prognostic value .
	manualset3
263772	11	426267	7	NULL	NULL	NULL	NULL	 prognostic value	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of NEFA levels in arterial and coronary sinus blood in patients with AMI and their temporal dynamics may be helpful for evaluation of the degree of the disease severity and can also be of prognostic value .
	manualset3
263778	1	426268	7	NULL	NULL	NULL	NULL	Determination	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of digoxin in human serum using stable isotope dilution liquid chromatography/electrospray ionization-tandem mass spectrometry .
	manualset3
263781	2	426268	7	NULL	NULL	NULL	NULL	digoxin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of digoxin in human serum using stable isotope dilution liquid chromatography/electrospray ionization-tandem mass spectrometry .
	manualset3
263783	3	426268	7	NULL	NULL	NULL	NULL	human serum 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of digoxin in human serum using stable isotope dilution liquid chromatography/electrospray ionization-tandem mass spectrometry .
	manualset3
263785	4	426268	7	NULL	NULL	NULL	NULL	stable isotope dilution liquid chromatography/electrospray ionization-tandem mass spectrometry	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of digoxin in human serum using stable isotope dilution liquid chromatography/electrospray ionization-tandem mass spectrometry .
	manualset3
263789	1	426269	7	NULL	NULL	NULL	NULL	Determination 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of guanfacine in biological fluids by electron-capture GLC .
	manualset3
263790	2	426269	7	NULL	NULL	NULL	NULL	guanfacine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of guanfacine in biological fluids by electron-capture GLC .
	manualset3
263791	3	426269	7	NULL	NULL	NULL	NULL	 biological fluids	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of guanfacine in biological fluids by electron-capture GLC .
	manualset3
263793	4	426269	7	NULL	NULL	NULL	NULL	 electron-capture GLC 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of guanfacine in biological fluids by electron-capture GLC .
	manualset3
263795	1	426270	7	NULL	NULL	NULL	NULL	Determination	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of lethium in microliter samples of blood serum using flame atomic emission spectrometry with a tantalum filament vaporizer .
	manualset3
263796	2	426270	7	NULL	NULL	NULL	NULL	lethium	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of lethium in microliter samples of blood serum using flame atomic emission spectrometry with a tantalum filament vaporizer .
	manualset3
263797	3	426270	7	NULL	NULL	NULL	NULL	microliter samples	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of lethium in microliter samples of blood serum using flame atomic emission spectrometry with a tantalum filament vaporizer .
	manualset3
263799	4	426270	7	NULL	NULL	NULL	NULL	 blood serum	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of lethium in microliter samples of blood serum using flame atomic emission spectrometry with a tantalum filament vaporizer .
	manualset3
263800	5	426270	7	NULL	NULL	NULL	NULL	flame atomic emission spectrometry	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of lethium in microliter samples of blood serum using flame atomic emission spectrometry with a tantalum filament vaporizer .
	manualset3
263801	6	426270	7	NULL	NULL	NULL	NULL	tantalum filament vaporizer	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of lethium in microliter samples of blood serum using flame atomic emission spectrometry with a tantalum filament vaporizer .
	manualset3
263802	1	426271	7	NULL	NULL	NULL	NULL	Determination	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of the binding sites of the proton transfer inhibitors Cd2 + and Zn2 + in bacterial reaction centers .
	manualset3
263804	2	426271	7	NULL	NULL	NULL	NULL	 binding sites 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of the binding sites of the proton transfer inhibitors Cd2 + and Zn2 + in bacterial reaction centers .
	manualset3
263805	3	426271	7	NULL	NULL	NULL	NULL	proton transfer inhibitors 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of the binding sites of the proton transfer inhibitors Cd2 + and Zn2 + in bacterial reaction centers .
	manualset3
263806	4	426271	7	NULL	NULL	NULL	NULL	Cd2 +	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of the binding sites of the proton transfer inhibitors Cd2 + and Zn2 + in bacterial reaction centers .
	manualset3
263807	5	426271	7	NULL	NULL	NULL	NULL	Zn2 +	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of the binding sites of the proton transfer inhibitors Cd2 + and Zn2 + in bacterial reaction centers .
	manualset3
263808	6	426271	7	NULL	NULL	NULL	NULL	bacterial reaction centers	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of the binding sites of the proton transfer inhibitors Cd2 + and Zn2 + in bacterial reaction centers .
	manualset3
263809	1	426272	7	NULL	NULL	NULL	NULL	Determination	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of the heme and protein portions of phenobarbital ( PB ) - inducible and 3-methylcholanthrene inducible forms of cytochrome P-450 , P-450 ( PB-1 ) , and P-450 ( MC-1 ) , in the liver microsomes of drug-treated animals indicated the presence of 20-30 % of apo-cytochrome P-450 in both cases .
	manualset3
263811	2	426272	7	NULL	NULL	NULL	NULL	heme portion	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of the heme and protein portions of phenobarbital ( PB ) - inducible and 3-methylcholanthrene inducible forms of cytochrome P-450 , P-450 ( PB-1 ) , and P-450 ( MC-1 ) , in the liver microsomes of drug-treated animals indicated the presence of 20-30 % of apo-cytochrome P-450 in both cases .
	manualset3
263812	3	426272	7	NULL	NULL	NULL	NULL	protein portions	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of the heme and protein portions of phenobarbital ( PB ) - inducible and 3-methylcholanthrene inducible forms of cytochrome P-450 , P-450 ( PB-1 ) , and P-450 ( MC-1 ) , in the liver microsomes of drug-treated animals indicated the presence of 20-30 % of apo-cytochrome P-450 in both cases .
	manualset3
263814	4	426272	7	NULL	NULL	NULL	NULL	phenobarbital ( PB ) - inducible forms	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of the heme and protein portions of phenobarbital ( PB ) - inducible and 3-methylcholanthrene inducible forms of cytochrome P-450 , P-450 ( PB-1 ) , and P-450 ( MC-1 ) , in the liver microsomes of drug-treated animals indicated the presence of 20-30 % of apo-cytochrome P-450 in both cases .
	manualset3
263815	5	426272	7	NULL	NULL	NULL	NULL	3-methylcholanthrene inducible forms	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of the heme and protein portions of phenobarbital ( PB ) - inducible and 3-methylcholanthrene inducible forms of cytochrome P-450 , P-450 ( PB-1 ) , and P-450 ( MC-1 ) , in the liver microsomes of drug-treated animals indicated the presence of 20-30 % of apo-cytochrome P-450 in both cases .
	manualset3
263816	6	426272	7	NULL	NULL	NULL	NULL	cytochrome P-450	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of the heme and protein portions of phenobarbital ( PB ) - inducible and 3-methylcholanthrene inducible forms of cytochrome P-450 , P-450 ( PB-1 ) , and P-450 ( MC-1 ) , in the liver microsomes of drug-treated animals indicated the presence of 20-30 % of apo-cytochrome P-450 in both cases .
	manualset3
263817	7	426272	7	NULL	NULL	NULL	NULL	P-450 ( PB-1 )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of the heme and protein portions of phenobarbital ( PB ) - inducible and 3-methylcholanthrene inducible forms of cytochrome P-450 , P-450 ( PB-1 ) , and P-450 ( MC-1 ) , in the liver microsomes of drug-treated animals indicated the presence of 20-30 % of apo-cytochrome P-450 in both cases .
	manualset3
263818	8	426272	7	NULL	NULL	NULL	NULL	P-450 ( MC-1 )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of the heme and protein portions of phenobarbital ( PB ) - inducible and 3-methylcholanthrene inducible forms of cytochrome P-450 , P-450 ( PB-1 ) , and P-450 ( MC-1 ) , in the liver microsomes of drug-treated animals indicated the presence of 20-30 % of apo-cytochrome P-450 in both cases .
	manualset3
263819	9	426272	7	NULL	NULL	NULL	NULL	liver microsomes 	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of the heme and protein portions of phenobarbital ( PB ) - inducible and 3-methylcholanthrene inducible forms of cytochrome P-450 , P-450 ( PB-1 ) , and P-450 ( MC-1 ) , in the liver microsomes of drug-treated animals indicated the presence of 20-30 % of apo-cytochrome P-450 in both cases .
	manualset3
263821	10	426272	7	NULL	NULL	NULL	NULL	drug-treated animals	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of the heme and protein portions of phenobarbital ( PB ) - inducible and 3-methylcholanthrene inducible forms of cytochrome P-450 , P-450 ( PB-1 ) , and P-450 ( MC-1 ) , in the liver microsomes of drug-treated animals indicated the presence of 20-30 % of apo-cytochrome P-450 in both cases .
	manualset3
263822	11	426272	7	NULL	NULL	NULL	NULL	presence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of the heme and protein portions of phenobarbital ( PB ) - inducible and 3-methylcholanthrene inducible forms of cytochrome P-450 , P-450 ( PB-1 ) , and P-450 ( MC-1 ) , in the liver microsomes of drug-treated animals indicated the presence of 20-30 % of apo-cytochrome P-450 in both cases .
	manualset3
263823	12	426272	7	NULL	NULL	NULL	NULL	 20-30 %	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of the heme and protein portions of phenobarbital ( PB ) - inducible and 3-methylcholanthrene inducible forms of cytochrome P-450 , P-450 ( PB-1 ) , and P-450 ( MC-1 ) , in the liver microsomes of drug-treated animals indicated the presence of 20-30 % of apo-cytochrome P-450 in both cases .
	manualset3
263824	13	426272	7	NULL	NULL	NULL	NULL	apo-cytochrome P-450	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of the heme and protein portions of phenobarbital ( PB ) - inducible and 3-methylcholanthrene inducible forms of cytochrome P-450 , P-450 ( PB-1 ) , and P-450 ( MC-1 ) , in the liver microsomes of drug-treated animals indicated the presence of 20-30 % of apo-cytochrome P-450 in both cases .
	manualset3
264039	14	426272	7	NULL	NULL	NULL	NULL	cases	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of the heme and protein portions of phenobarbital ( PB ) - inducible and 3-methylcholanthrene inducible forms of cytochrome P-450 , P-450 ( PB-1 ) , and P-450 ( MC-1 ) , in the liver microsomes of drug-treated animals indicated the presence of 20-30 % of apo-cytochrome P-450 in both cases .
	manualset3
264040	1	426273	7	NULL	NULL	NULL	NULL	Determination	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of the location of intron/exon boundaries in the Lmp-2 gene indicated that these residues correspond precisely to the first exon of the gene .
	manualset3
264041	2	426273	7	NULL	NULL	NULL	NULL	 location	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of the location of intron/exon boundaries in the Lmp-2 gene indicated that these residues correspond precisely to the first exon of the gene .
	manualset3
264042	3	426273	7	NULL	NULL	NULL	NULL	intron/exon boundaries	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of the location of intron/exon boundaries in the Lmp-2 gene indicated that these residues correspond precisely to the first exon of the gene .
	manualset3
264043	4	426273	7	NULL	NULL	NULL	NULL	Lmp-2 gene	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of the location of intron/exon boundaries in the Lmp-2 gene indicated that these residues correspond precisely to the first exon of the gene .
	manualset3
264044	5	426273	7	NULL	NULL	NULL	NULL	residues	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of the location of intron/exon boundaries in the Lmp-2 gene indicated that these residues correspond precisely to the first exon of the gene .
	manualset3
264045	6	426273	7	NULL	NULL	NULL	NULL	first exon	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of the location of intron/exon boundaries in the Lmp-2 gene indicated that these residues correspond precisely to the first exon of the gene .
	manualset3
264046	7	426273	7	NULL	NULL	NULL	NULL	gene 	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determination of the location of intron/exon boundaries in the Lmp-2 gene indicated that these residues correspond precisely to the first exon of the gene .
	manualset3
264047	1	426274	7	NULL	NULL	NULL	NULL	Nitrogen use efficiency	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Nitrogen use efficiency and its relationship with nitrogen nutrition characteristics of wheat varieties ) .
	manualset3
264048	2	426274	7	NULL	NULL	NULL	NULL	relationship	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Nitrogen use efficiency and its relationship with nitrogen nutrition characteristics of wheat varieties ) .
	manualset3
264049	3	426274	7	NULL	NULL	NULL	NULL	nitrogen nutrition 	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Nitrogen use efficiency and its relationship with nitrogen nutrition characteristics of wheat varieties ) .
	manualset3
264050	4	426274	7	NULL	NULL	NULL	NULL	wheat varieties 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Nitrogen use efficiency and its relationship with nitrogen nutrition characteristics of wheat varieties ) .
	manualset3
264051	1	426275	7	NULL	NULL	NULL	NULL	Determinations	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determinations of specific immunoglobulin E were carried out with HSA-DGEBA conjugates , two DGEBA-based epoxy resins , and phthalic anhydrides .
	manualset3
264052	2	426275	7	NULL	NULL	NULL	NULL	specific immunoglobulin E	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determinations of specific immunoglobulin E were carried out with HSA-DGEBA conjugates , two DGEBA-based epoxy resins , and phthalic anhydrides .
	manualset3
264053	3	426275	7	NULL	NULL	NULL	NULL	HSA-DGEBA conjugates	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determinations of specific immunoglobulin E were carried out with HSA-DGEBA conjugates , two DGEBA-based epoxy resins , and phthalic anhydrides .
	manualset3
264054	4	426275	7	NULL	NULL	NULL	NULL	two DGEBA-based epoxy resins	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determinations of specific immunoglobulin E were carried out with HSA-DGEBA conjugates , two DGEBA-based epoxy resins , and phthalic anhydrides .
	manualset3
264055	5	426275	7	NULL	NULL	NULL	NULL	phthalic anhydrides	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determinations of specific immunoglobulin E were carried out with HSA-DGEBA conjugates , two DGEBA-based epoxy resins , and phthalic anhydrides .
	manualset3
264056	1	426276	7	NULL	NULL	NULL	NULL	Determinations	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determinations were made of the inhibitory activities of four benzimidazoles and six recently synthesised pyrimidine derivatives on the SOD enzymes from the cestodes .
	manualset3
264057	2	426276	7	NULL	NULL	NULL	NULL	inhibitory activities	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determinations were made of the inhibitory activities of four benzimidazoles and six recently synthesised pyrimidine derivatives on the SOD enzymes from the cestodes .
	manualset3
264058	3	426276	7	NULL	NULL	NULL	NULL	 four benzimidazoles 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determinations were made of the inhibitory activities of four benzimidazoles and six recently synthesised pyrimidine derivatives on the SOD enzymes from the cestodes .
	manualset3
264059	4	426276	7	NULL	NULL	NULL	NULL	 six 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determinations were made of the inhibitory activities of four benzimidazoles and six recently synthesised pyrimidine derivatives on the SOD enzymes from the cestodes .
	manualset3
264060	5	426276	7	NULL	NULL	NULL	NULL	pyrimidine derivatives	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determinations were made of the inhibitory activities of four benzimidazoles and six recently synthesised pyrimidine derivatives on the SOD enzymes from the cestodes .
	manualset3
264061	6	426276	7	NULL	NULL	NULL	NULL	SOD enzymes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determinations were made of the inhibitory activities of four benzimidazoles and six recently synthesised pyrimidine derivatives on the SOD enzymes from the cestodes .
	manualset3
264062	7	426276	7	NULL	NULL	NULL	NULL	cestodes	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determinations were made of the inhibitory activities of four benzimidazoles and six recently synthesised pyrimidine derivatives on the SOD enzymes from the cestodes .
	manualset3
264063	1	426277	7	NULL	NULL	NULL	NULL	optimum hemoglobin sampling	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determining optimum hemoglobin sampling for anemia management from every-treatment data .
	manualset3
264064	2	426277	7	NULL	NULL	NULL	NULL	 anemia management	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determining optimum hemoglobin sampling for anemia management from every-treatment data .
	manualset3
264065	3	426277	7	NULL	NULL	NULL	NULL	 every-treatment data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determining optimum hemoglobin sampling for anemia management from every-treatment data .
	manualset3
264066	1	426278	7	NULL	NULL	NULL	NULL	potential indicators	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determining potential indicators of Cryptosporidium oocysts throughout the wastewater treatment process .
	manualset3
264067	2	426278	7	NULL	NULL	NULL	NULL	Cryptosporidium oocysts	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determining potential indicators of Cryptosporidium oocysts throughout the wastewater treatment process .
	manualset3
264068	3	426278	7	NULL	NULL	NULL	NULL	wastewater treatment process	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determining potential indicators of Cryptosporidium oocysts throughout the wastewater treatment process .
	manualset3
264069	1	426279	7	NULL	NULL	NULL	NULL	 length 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determining the length of hospital stay on the basis of infarction size is justified .
	manualset3
264070	2	426279	7	NULL	NULL	NULL	NULL	hospital stay 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determining the length of hospital stay on the basis of infarction size is justified .
	manualset3
264071	3	426279	7	NULL	NULL	NULL	NULL	basis	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determining the length of hospital stay on the basis of infarction size is justified .
	manualset3
264072	4	426279	7	NULL	NULL	NULL	NULL	 infarction size	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Determining the length of hospital stay on the basis of infarction size is justified .
	manualset3
264073	2	426280	7	NULL	NULL	NULL	NULL	 alcohol consumption	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Developing a genetically informative measure of alcohol consumption using past-12-month indices .
	manualset3
264074	1	426280	7	NULL	NULL	NULL	NULL	genetically informative measure	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Developing a genetically informative measure of alcohol consumption using past-12-month indices .
	manualset3
264075	3	426280	7	NULL	NULL	NULL	NULL	 past-12-month indices	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Developing a genetically informative measure of alcohol consumption using past-12-month indices .
	manualset3
264076	1	426281	7	NULL	NULL	NULL	NULL	pancreatic cancer specific promoter ( PCSP )	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Developing a pancreatic cancer specific promoter ( PCSP ) is one approach for pancreatic cancer gene therapy .
	manualset3
264077	2	426281	7	NULL	NULL	NULL	NULL	one approach	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Developing a pancreatic cancer specific promoter ( PCSP ) is one approach for pancreatic cancer gene therapy .
	manualset3
264078	3	426281	7	NULL	NULL	NULL	NULL	 pancreatic cancer gene therapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Developing a pancreatic cancer specific promoter ( PCSP ) is one approach for pancreatic cancer gene therapy .
	manualset3
264079	1	426282	7	NULL	NULL	NULL	NULL	 hope	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Developing and maintaining hope in families of the critically ill .
	manualset3
264080	2	426282	7	NULL	NULL	NULL	NULL	families	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Developing and maintaining hope in families of the critically ill .
	manualset3
264081	3	426282	7	NULL	NULL	NULL	NULL	critically ill	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Developing and maintaining hope in families of the critically ill .
	manualset3
264082	1	426283	7	NULL	NULL	NULL	NULL	risk models	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Developing risk models of Cryptosporidium transport in soils from vegetated , tilted soilbox experiments .
	manualset3
264083	2	426283	7	NULL	NULL	NULL	NULL	Cryptosporidium transport	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Developing risk models of Cryptosporidium transport in soils from vegetated , tilted soilbox experiments .
	manualset3
264084	3	426283	7	NULL	NULL	NULL	NULL	soils	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Developing risk models of Cryptosporidium transport in soils from vegetated , tilted soilbox experiments .
	manualset3
264085	4	426283	7	NULL	NULL	NULL	NULL	 vegetated , tilted soilbox experiments	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Developing risk models of Cryptosporidium transport in soils from vegetated , tilted soilbox experiments .
	manualset3
264086	1	426284	7	NULL	NULL	NULL	NULL	Development	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of WAIS-III General Ability Index Minus WMS-III memory discrepancy scores .
	manualset3
264087	2	426284	7	NULL	NULL	NULL	NULL	WAIS-III General Ability Index Minus WMS-III memory discrepancy scores	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of WAIS-III General Ability Index Minus WMS-III memory discrepancy scores .
	manualset3
264088	1	426285	7	NULL	NULL	NULL	NULL	Development 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development and evaluation in an ex vivo rat model of a technique for the endoscopic assessment of mucosal defense in man .
	manualset3
264089	2	426285	7	NULL	NULL	NULL	NULL	evaluation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development and evaluation in an ex vivo rat model of a technique for the endoscopic assessment of mucosal defense in man .
	manualset3
264090	3	426285	7	NULL	NULL	NULL	NULL	ex vivo rat model	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development and evaluation in an ex vivo rat model of a technique for the endoscopic assessment of mucosal defense in man .
	manualset3
264091	4	426285	7	NULL	NULL	NULL	NULL	technique	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development and evaluation in an ex vivo rat model of a technique for the endoscopic assessment of mucosal defense in man .
	manualset3
264092	5	426285	7	NULL	NULL	NULL	NULL	 endoscopic assessment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development and evaluation in an ex vivo rat model of a technique for the endoscopic assessment of mucosal defense in man .
	manualset3
264093	6	426285	7	NULL	NULL	NULL	NULL	mucosal defense	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development and evaluation in an ex vivo rat model of a technique for the endoscopic assessment of mucosal defense in man .
	manualset3
264094	7	426285	7	NULL	NULL	NULL	NULL	man	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development and evaluation in an ex vivo rat model of a technique for the endoscopic assessment of mucosal defense in man .
	manualset3
264095	1	426286	7	NULL	NULL	NULL	NULL	Development	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development and functions of natural killer cells .
	manualset3
264096	2	426286	7	NULL	NULL	NULL	NULL	functions	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development and functions of natural killer cells .
	manualset3
264097	3	426286	7	NULL	NULL	NULL	NULL	natural killer cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development and functions of natural killer cells .
	manualset3
264098	1	426287	7	NULL	NULL	NULL	NULL	Development	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development and validation of a BEAMnrc component module for a miniature multileaf collimator .
	manualset3
264099	2	426287	7	NULL	NULL	NULL	NULL	validation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development and validation of a BEAMnrc component module for a miniature multileaf collimator .
	manualset3
264100	3	426287	7	NULL	NULL	NULL	NULL	BEAMnrc component module	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development and validation of a BEAMnrc component module for a miniature multileaf collimator .
	manualset3
264101	4	426287	7	NULL	NULL	NULL	NULL	miniature multileaf collimator	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development and validation of a BEAMnrc component module for a miniature multileaf collimator .
	manualset3
264102	1	426288	7	NULL	NULL	NULL	NULL	Development 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development and validation of a novel competitive ELISA for the detection of serum amyloid A in pigs .
	manualset3
264103	2	426288	7	NULL	NULL	NULL	NULL	validation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development and validation of a novel competitive ELISA for the detection of serum amyloid A in pigs .
	manualset3
264104	3	426288	7	NULL	NULL	NULL	NULL	novel competitive ELISA 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development and validation of a novel competitive ELISA for the detection of serum amyloid A in pigs .
	manualset3
264105	4	426288	7	NULL	NULL	NULL	NULL	detection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development and validation of a novel competitive ELISA for the detection of serum amyloid A in pigs .
	manualset3
264106	5	426288	7	NULL	NULL	NULL	NULL	serum amyloid A	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development and validation of a novel competitive ELISA for the detection of serum amyloid A in pigs .
	manualset3
264107	6	426288	7	NULL	NULL	NULL	NULL	pigs 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development and validation of a novel competitive ELISA for the detection of serum amyloid A in pigs .
	manualset3
264108	1	426289	7	NULL	NULL	NULL	NULL	Development	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of a monoclonal antibody capable of differentiating platelet PLA1/PLA1 , PLA1/PLA2 and PLA2/PLA2 genotypes .
	manualset3
264109	2	426289	7	NULL	NULL	NULL	NULL	monoclonal antibody	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of a monoclonal antibody capable of differentiating platelet PLA1/PLA1 , PLA1/PLA2 and PLA2/PLA2 genotypes .
	manualset3
264110	3	426289	7	NULL	NULL	NULL	NULL	 platelet PLA1/PLA1 genotypes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of a monoclonal antibody capable of differentiating platelet PLA1/PLA1 , PLA1/PLA2 and PLA2/PLA2 genotypes .
	manualset3
264111	4	426289	7	NULL	NULL	NULL	NULL	PLA1/PLA2 genotype	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of a monoclonal antibody capable of differentiating platelet PLA1/PLA1 , PLA1/PLA2 and PLA2/PLA2 genotypes .
	manualset3
264112	5	426289	7	NULL	NULL	NULL	NULL	PLA2/PLA2 genotypes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of a monoclonal antibody capable of differentiating platelet PLA1/PLA1 , PLA1/PLA2 and PLA2/PLA2 genotypes .
	manualset3
264113	1	426290	7	NULL	NULL	NULL	NULL	Non-invasive assessment	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Non-invasive assessment of coronary reperfusion ) .
	manualset3
264114	2	426290	7	NULL	NULL	NULL	NULL	coronary reperfusion	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Non-invasive assessment of coronary reperfusion ) .
	manualset3
264115	1	426291	7	NULL	NULL	NULL	NULL	Development	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of a regional trauma center : nursing approach .
	manualset3
264116	2	426291	7	NULL	NULL	NULL	NULL	regional trauma center	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of a regional trauma center : nursing approach .
	manualset3
264117	3	426291	7	NULL	NULL	NULL	NULL	nursing approach	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of a regional trauma center : nursing approach .
	manualset3
264118	1	426292	7	NULL	NULL	NULL	NULL	Development	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of an instrument to measure health center ( HC ) personnel 's computer use , knowledge and functionality demand for HC computerized information system in Thailand .
	manualset3
264119	2	426292	7	NULL	NULL	NULL	NULL	 instrument	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of an instrument to measure health center ( HC ) personnel 's computer use , knowledge and functionality demand for HC computerized information system in Thailand .
	manualset3
264120	3	426292	7	NULL	NULL	NULL	NULL	health center ( HC ) personnel 's computer use	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of an instrument to measure health center ( HC ) personnel 's computer use , knowledge and functionality demand for HC computerized information system in Thailand .
	manualset3
264121	4	426292	7	NULL	NULL	NULL	NULL	knowledge	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of an instrument to measure health center ( HC ) personnel 's computer use , knowledge and functionality demand for HC computerized information system in Thailand .
	manualset3
264122	5	426292	7	NULL	NULL	NULL	NULL	 functionality demand	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of an instrument to measure health center ( HC ) personnel 's computer use , knowledge and functionality demand for HC computerized information system in Thailand .
	manualset3
264123	6	426292	7	NULL	NULL	NULL	NULL	HC computerized information system	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of an instrument to measure health center ( HC ) personnel 's computer use , knowledge and functionality demand for HC computerized information system in Thailand .
	manualset3
264124	7	426292	7	NULL	NULL	NULL	NULL	Thailand	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of an instrument to measure health center ( HC ) personnel 's computer use , knowledge and functionality demand for HC computerized information system in Thailand .
	manualset3
264125	1	426293	7	NULL	NULL	NULL	NULL	Development	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of biological parameters and therapeutic recommendations ) .
	manualset3
264126	2	426293	7	NULL	NULL	NULL	NULL	biological parameters 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of biological parameters and therapeutic recommendations ) .
	manualset3
264127	3	426293	7	NULL	NULL	NULL	NULL	therapeutic recommendations	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of biological parameters and therapeutic recommendations ) .
	manualset3
264128	1	426294	7	NULL	NULL	NULL	NULL	Development	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of electrical rhythmicity in the murine gastrointestinal tract is specifically encoded in the tunica muscularis .
	manualset3
264129	2	426294	7	NULL	NULL	NULL	NULL	electrical rhythmicity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of electrical rhythmicity in the murine gastrointestinal tract is specifically encoded in the tunica muscularis .
	manualset3
264130	3	426294	7	NULL	NULL	NULL	NULL	murine gastrointestinal tract	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of electrical rhythmicity in the murine gastrointestinal tract is specifically encoded in the tunica muscularis .
	manualset3
264131	4	426294	7	NULL	NULL	NULL	NULL	tunica muscularis	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of electrical rhythmicity in the murine gastrointestinal tract is specifically encoded in the tunica muscularis .
	manualset3
264132	1	426295	7	NULL	NULL	NULL	NULL	Development	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of mouse limb buds in organ culture : chondrogenesis in the presence of a proline analog , L-azetidine-2-carboxylic acid .
	manualset3
264133	2	426295	7	NULL	NULL	NULL	NULL	mouse limb buds	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of mouse limb buds in organ culture : chondrogenesis in the presence of a proline analog , L-azetidine-2-carboxylic acid .
	manualset3
264134	3	426295	7	NULL	NULL	NULL	NULL	organ culture	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of mouse limb buds in organ culture : chondrogenesis in the presence of a proline analog , L-azetidine-2-carboxylic acid .
	manualset3
264135	4	426295	7	NULL	NULL	NULL	NULL	chondrogenesis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of mouse limb buds in organ culture : chondrogenesis in the presence of a proline analog , L-azetidine-2-carboxylic acid .
	manualset3
264136	5	426295	7	NULL	NULL	NULL	NULL	presence	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of mouse limb buds in organ culture : chondrogenesis in the presence of a proline analog , L-azetidine-2-carboxylic acid .
	manualset3
264137	6	426295	7	NULL	NULL	NULL	NULL	proline analog	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of mouse limb buds in organ culture : chondrogenesis in the presence of a proline analog , L-azetidine-2-carboxylic acid .
	manualset3
264138	7	426295	7	NULL	NULL	NULL	NULL	L-azetidine-2-carboxylic acid	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of mouse limb buds in organ culture : chondrogenesis in the presence of a proline analog , L-azetidine-2-carboxylic acid .
	manualset3
264139	1	426296	7	NULL	NULL	NULL	NULL	Development	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of physical response after athletics training in adolescents with Down 's syndrome .
	manualset3
264140	2	426296	7	NULL	NULL	NULL	NULL	physical response	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of physical response after athletics training in adolescents with Down 's syndrome .
	manualset3
264141	3	426296	7	NULL	NULL	NULL	NULL	athletics training	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of physical response after athletics training in adolescents with Down 's syndrome .
	manualset3
264142	4	426296	7	NULL	NULL	NULL	NULL	adolescents	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of physical response after athletics training in adolescents with Down 's syndrome .
	manualset3
264143	5	426296	7	NULL	NULL	NULL	NULL	Down 's syndrome	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of physical response after athletics training in adolescents with Down 's syndrome .
	manualset3
264144	1	426297	7	NULL	NULL	NULL	NULL	Development 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of still more powerful computer hardware and software will enable extensive studies of the protein structure and dynamics of new potential drug targets , but raises a new challenge in the validation and calibration of computerized methods of biosimulations .
	manualset3
264145	2	426297	7	NULL	NULL	NULL	NULL	 powerful computer hardware	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of still more powerful computer hardware and software will enable extensive studies of the protein structure and dynamics of new potential drug targets , but raises a new challenge in the validation and calibration of computerized methods of biosimulations .
	manualset3
264146	3	426297	7	NULL	NULL	NULL	NULL	software	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of still more powerful computer hardware and software will enable extensive studies of the protein structure and dynamics of new potential drug targets , but raises a new challenge in the validation and calibration of computerized methods of biosimulations .
	manualset3
264147	4	426297	7	NULL	NULL	NULL	NULL	extensive studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of still more powerful computer hardware and software will enable extensive studies of the protein structure and dynamics of new potential drug targets , but raises a new challenge in the validation and calibration of computerized methods of biosimulations .
	manualset3
264148	5	426297	7	NULL	NULL	NULL	NULL	protein structure	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of still more powerful computer hardware and software will enable extensive studies of the protein structure and dynamics of new potential drug targets , but raises a new challenge in the validation and calibration of computerized methods of biosimulations .
	manualset3
264149	6	426297	7	NULL	NULL	NULL	NULL	dynamics	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of still more powerful computer hardware and software will enable extensive studies of the protein structure and dynamics of new potential drug targets , but raises a new challenge in the validation and calibration of computerized methods of biosimulations .
	manualset3
264150	7	426297	7	NULL	NULL	NULL	NULL	new potential drug targets	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of still more powerful computer hardware and software will enable extensive studies of the protein structure and dynamics of new potential drug targets , but raises a new challenge in the validation and calibration of computerized methods of biosimulations .
	manualset3
264151	8	426297	7	NULL	NULL	NULL	NULL	challenge 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of still more powerful computer hardware and software will enable extensive studies of the protein structure and dynamics of new potential drug targets , but raises a new challenge in the validation and calibration of computerized methods of biosimulations .
	manualset3
264152	9	426297	7	NULL	NULL	NULL	NULL	 validation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of still more powerful computer hardware and software will enable extensive studies of the protein structure and dynamics of new potential drug targets , but raises a new challenge in the validation and calibration of computerized methods of biosimulations .
	manualset3
264153	10	426297	7	NULL	NULL	NULL	NULL	calibration 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of still more powerful computer hardware and software will enable extensive studies of the protein structure and dynamics of new potential drug targets , but raises a new challenge in the validation and calibration of computerized methods of biosimulations .
	manualset3
264154	11	426297	7	NULL	NULL	NULL	NULL	 computerized methods 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of still more powerful computer hardware and software will enable extensive studies of the protein structure and dynamics of new potential drug targets , but raises a new challenge in the validation and calibration of computerized methods of biosimulations .
	manualset3
264155	12	426297	7	NULL	NULL	NULL	NULL	biosimulations	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of still more powerful computer hardware and software will enable extensive studies of the protein structure and dynamics of new potential drug targets , but raises a new challenge in the validation and calibration of computerized methods of biosimulations .
	manualset3
264156	1	426298	7	NULL	NULL	NULL	NULL	Development	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of the rat phrenic nucleus and its connections with brainstem respiratory nuclei .
	manualset3
264157	2	426298	7	NULL	NULL	NULL	NULL	 rat phrenic nucleus	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of the rat phrenic nucleus and its connections with brainstem respiratory nuclei .
	manualset3
264158	3	426298	7	NULL	NULL	NULL	NULL	connections	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of the rat phrenic nucleus and its connections with brainstem respiratory nuclei .
	manualset3
264159	4	426298	7	NULL	NULL	NULL	NULL	brainstem respiratory nuclei	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Development of the rat phrenic nucleus and its connections with brainstem respiratory nuclei .
	manualset3
264160	1	426299	7	NULL	NULL	NULL	NULL	Developmental delay	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Developmental delay and dysmorphic features associated with a previously undescribed deletion on chromosome 1 .
	manualset3
264161	2	426299	7	NULL	NULL	NULL	NULL	dysmorphic features 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Developmental delay and dysmorphic features associated with a previously undescribed deletion on chromosome 1 .
	manualset3
264162	3	426299	7	NULL	NULL	NULL	NULL	deletion	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Developmental delay and dysmorphic features associated with a previously undescribed deletion on chromosome 1 .
	manualset3
264163	4	426299	7	NULL	NULL	NULL	NULL	chromosome 1	Chromosome												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Developmental delay and dysmorphic features associated with a previously undescribed deletion on chromosome 1 .
	manualset3
264164	1	426300	7	NULL	NULL	NULL	NULL	Noninvasive method 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Noninvasive method of determining the cerebral blood flow circulation rate and its correlations with cardiac minute volume ) .
	manualset3
264165	2	426300	7	NULL	NULL	NULL	NULL	cerebral blood flow circulation rate	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Noninvasive method of determining the cerebral blood flow circulation rate and its correlations with cardiac minute volume ) .
	manualset3
264166	3	426300	7	NULL	NULL	NULL	NULL	 correlations	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Noninvasive method of determining the cerebral blood flow circulation rate and its correlations with cardiac minute volume ) .
	manualset3
264167	4	426300	7	NULL	NULL	NULL	NULL	cardiac minute volume	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Noninvasive method of determining the cerebral blood flow circulation rate and its correlations with cardiac minute volume ) .
	manualset3
264168	1	426301	7	NULL	NULL	NULL	NULL	Developmental expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Developmental expression of rat insulin-like growth factor binding protein-2 by astrocytic glial cells in culture .
	manualset3
264169	2	426301	7	NULL	NULL	NULL	NULL	rat insulin-like growth factor binding protein-2	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Developmental expression of rat insulin-like growth factor binding protein-2 by astrocytic glial cells in culture .
	manualset3
264170	3	426301	7	NULL	NULL	NULL	NULL	 astrocytic glial cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Developmental expression of rat insulin-like growth factor binding protein-2 by astrocytic glial cells in culture .
	manualset3
264171	4	426301	7	NULL	NULL	NULL	NULL	culture	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Developmental expression of rat insulin-like growth factor binding protein-2 by astrocytic glial cells in culture .
	manualset3
264172	1	426302	7	NULL	NULL	NULL	NULL	Developmental plasticity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Developmental plasticity , morphological variation and evolvability : a multilevel analysis of morphometric integration in the shape of compound leaves .
	manualset3
264173	2	426302	7	NULL	NULL	NULL	NULL	morphological variation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Developmental plasticity , morphological variation and evolvability : a multilevel analysis of morphometric integration in the shape of compound leaves .
	manualset3
264174	3	426302	7	NULL	NULL	NULL	NULL	evolvability	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Developmental plasticity , morphological variation and evolvability : a multilevel analysis of morphometric integration in the shape of compound leaves .
	manualset3
264175	4	426302	7	NULL	NULL	NULL	NULL	multilevel analysis	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Developmental plasticity , morphological variation and evolvability : a multilevel analysis of morphometric integration in the shape of compound leaves .
	manualset3
264176	5	426302	7	NULL	NULL	NULL	NULL	morphometric integration	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Developmental plasticity , morphological variation and evolvability : a multilevel analysis of morphometric integration in the shape of compound leaves .
	manualset3
264177	6	426302	7	NULL	NULL	NULL	NULL	 shape	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Developmental plasticity , morphological variation and evolvability : a multilevel analysis of morphometric integration in the shape of compound leaves .
	manualset3
264178	7	426302	7	NULL	NULL	NULL	NULL	compound leaves 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Developmental plasticity , morphological variation and evolvability : a multilevel analysis of morphometric integration in the shape of compound leaves .
	manualset3
264179	1	426303	7	NULL	NULL	NULL	NULL	Dexamethasone-induced protein degradation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dexamethasone-induced protein degradation in cultured myotubes is p300/HAT dependent .
	manualset3
264180	2	426303	7	NULL	NULL	NULL	NULL	cultured myotubes	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dexamethasone-induced protein degradation in cultured myotubes is p300/HAT dependent .
	manualset3
264181	3	426303	7	NULL	NULL	NULL	NULL	p300/HAT	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dexamethasone-induced protein degradation in cultured myotubes is p300/HAT dependent .
	manualset3
264182	1	426304	7	NULL	NULL	NULL	NULL	DiGeorge syndrome	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DiGeorge syndrome , Tbx1 , and retinoic acid signaling come full circle .
	manualset3
264183	2	426304	7	NULL	NULL	NULL	NULL	Tbx1	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DiGeorge syndrome , Tbx1 , and retinoic acid signaling come full circle .
	manualset3
264184	3	426304	7	NULL	NULL	NULL	NULL	 retinoic acid signaling	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DiGeorge syndrome , Tbx1 , and retinoic acid signaling come full circle .
	manualset3
264185	4	426304	7	NULL	NULL	NULL	NULL	 full circle	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DiGeorge syndrome , Tbx1 , and retinoic acid signaling come full circle .
	manualset3
264186	1	426305	7	NULL	NULL	NULL	NULL	DiI tracing 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DiI tracing of retinofugal pathways following uniocular injection demonstrated their bilateral localization and extensive termination in the diencephalon and mesencephalon of both sides .
	manualset3
264187	2	426305	7	NULL	NULL	NULL	NULL	retinofugal pathways	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DiI tracing of retinofugal pathways following uniocular injection demonstrated their bilateral localization and extensive termination in the diencephalon and mesencephalon of both sides .
	manualset3
264188	3	426305	7	NULL	NULL	NULL	NULL	uniocular injection	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DiI tracing of retinofugal pathways following uniocular injection demonstrated their bilateral localization and extensive termination in the diencephalon and mesencephalon of both sides .
	manualset3
264189	4	426305	7	NULL	NULL	NULL	NULL	 bilateral localization	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DiI tracing of retinofugal pathways following uniocular injection demonstrated their bilateral localization and extensive termination in the diencephalon and mesencephalon of both sides .
	manualset3
264190	5	426305	7	NULL	NULL	NULL	NULL	extensive termination	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DiI tracing of retinofugal pathways following uniocular injection demonstrated their bilateral localization and extensive termination in the diencephalon and mesencephalon of both sides .
	manualset3
264191	6	426305	7	NULL	NULL	NULL	NULL	 diencephalon 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DiI tracing of retinofugal pathways following uniocular injection demonstrated their bilateral localization and extensive termination in the diencephalon and mesencephalon of both sides .
	manualset3
264192	7	426305	7	NULL	NULL	NULL	NULL	mesencephalon	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DiI tracing of retinofugal pathways following uniocular injection demonstrated their bilateral localization and extensive termination in the diencephalon and mesencephalon of both sides .
	manualset3
264193	8	426305	7	NULL	NULL	NULL	NULL	sides	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DiI tracing of retinofugal pathways following uniocular injection demonstrated their bilateral localization and extensive termination in the diencephalon and mesencephalon of both sides .
	manualset3
264194	1	426306	7	NULL	NULL	NULL	NULL	Diabetes insipidus 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diabetes insipidus is a well-recognized complication of Langerhans-cell histiocytosis ( histiocytosis X ) , but its frequency and natural history are not well defined .
	manualset3
264195	2	426306	7	NULL	NULL	NULL	NULL	complication	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diabetes insipidus is a well-recognized complication of Langerhans-cell histiocytosis ( histiocytosis X ) , but its frequency and natural history are not well defined .
	manualset3
264196	3	426306	7	NULL	NULL	NULL	NULL	Langerhans-cell histiocytosis ( histiocytosis X )	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diabetes insipidus is a well-recognized complication of Langerhans-cell histiocytosis ( histiocytosis X ) , but its frequency and natural history are not well defined .
	manualset3
264197	4	426306	7	NULL	NULL	NULL	NULL	 frequency	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diabetes insipidus is a well-recognized complication of Langerhans-cell histiocytosis ( histiocytosis X ) , but its frequency and natural history are not well defined .
	manualset3
264198	5	426306	7	NULL	NULL	NULL	NULL	natural history	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diabetes insipidus is a well-recognized complication of Langerhans-cell histiocytosis ( histiocytosis X ) , but its frequency and natural history are not well defined .
	manualset3
264199	1	426307	7	NULL	NULL	NULL	NULL	Diabetes mellitus	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diabetes mellitus is a disease characterized by impaired glucose metabolism that leads to retinopathy , brain micro-infarcts and other complications .
	manualset3
264200	2	426307	7	NULL	NULL	NULL	NULL	disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diabetes mellitus is a disease characterized by impaired glucose metabolism that leads to retinopathy , brain micro-infarcts and other complications .
	manualset3
264201	3	426307	7	NULL	NULL	NULL	NULL	impaired glucose metabolism	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diabetes mellitus is a disease characterized by impaired glucose metabolism that leads to retinopathy , brain micro-infarcts and other complications .
	manualset3
264202	4	426307	7	NULL	NULL	NULL	NULL	 retinopathy	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diabetes mellitus is a disease characterized by impaired glucose metabolism that leads to retinopathy , brain micro-infarcts and other complications .
	manualset3
264203	5	426307	7	NULL	NULL	NULL	NULL	 brain micro-infarcts	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diabetes mellitus is a disease characterized by impaired glucose metabolism that leads to retinopathy , brain micro-infarcts and other complications .
	manualset3
264204	6	426307	7	NULL	NULL	NULL	NULL	complications	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diabetes mellitus is a disease characterized by impaired glucose metabolism that leads to retinopathy , brain micro-infarcts and other complications .
	manualset3
264205	1	426308	7	NULL	NULL	NULL	NULL	Diabetes	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diabetes , the ice free corridor , and the Paleoindian settlement of North America .
	manualset3
264206	2	426308	7	NULL	NULL	NULL	NULL	 ice free corridor	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diabetes , the ice free corridor , and the Paleoindian settlement of North America .
	manualset3
264207	3	426308	7	NULL	NULL	NULL	NULL	Paleoindian settlement	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diabetes , the ice free corridor , and the Paleoindian settlement of North America .
	manualset3
264208	4	426308	7	NULL	NULL	NULL	NULL	North America	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diabetes , the ice free corridor , and the Paleoindian settlement of North America .
	manualset3
264209	1	426309	7	NULL	NULL	NULL	NULL	Diabetes management	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diabetes management in long-term care facilities : a practical guide .
	manualset3
264210	2	426309	7	NULL	NULL	NULL	NULL	long-term care facilities	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diabetes management in long-term care facilities : a practical guide .
	manualset3
264211	3	426309	7	NULL	NULL	NULL	NULL	practical guide	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diabetes management in long-term care facilities : a practical guide .
	manualset3
264212	1	426310	7	NULL	NULL	NULL	NULL	Diagnosis 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis may be confusing in childhood , especially in the presence of neurofibromatosis when it must be differentiated from optic nerve glioma .
	manualset3
264213	2	426310	7	NULL	NULL	NULL	NULL	 childhood	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis may be confusing in childhood , especially in the presence of neurofibromatosis when it must be differentiated from optic nerve glioma .
	manualset3
264214	3	426310	7	NULL	NULL	NULL	NULL	presence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis may be confusing in childhood , especially in the presence of neurofibromatosis when it must be differentiated from optic nerve glioma .
	manualset3
264215	4	426310	7	NULL	NULL	NULL	NULL	neurofibromatosis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis may be confusing in childhood , especially in the presence of neurofibromatosis when it must be differentiated from optic nerve glioma .
	manualset3
264216	5	426310	7	NULL	NULL	NULL	NULL	optic nerve glioma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis may be confusing in childhood , especially in the presence of neurofibromatosis when it must be differentiated from optic nerve glioma .
	manualset3
264476	1	426311	7	NULL	NULL	NULL	NULL	Diagnosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis must exclude all other possible forms of oedema .
	manualset3
264479	2	426311	7	NULL	NULL	NULL	NULL	possible forms	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis must exclude all other possible forms of oedema .
	manualset3
264480	3	426311	7	NULL	NULL	NULL	NULL	oedema	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis must exclude all other possible forms of oedema .
	manualset3
264484	1	426312	7	NULL	NULL	NULL	NULL	Diagnosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis should be confirmed by fine-needle aspiration biopsy .
	manualset3
264485	2	426312	7	NULL	NULL	NULL	NULL	fine-needle aspiration biopsy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis should be confirmed by fine-needle aspiration biopsy .
	manualset3
264489	1	426313	7	NULL	NULL	NULL	NULL	Diagnosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis and management of cluster headaches .
	manualset3
264490	2	426313	7	NULL	NULL	NULL	NULL	management 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis and management of cluster headaches .
	manualset3
264493	3	426313	7	NULL	NULL	NULL	NULL	cluster headaches 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis and management of cluster headaches .
	manualset3
264499	1	426314	7	NULL	NULL	NULL	NULL	Diagnosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis and management of constipation and encopresis in childhood .
	manualset3
264501	2	426314	7	NULL	NULL	NULL	NULL	management 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis and management of constipation and encopresis in childhood .
	manualset3
264504	3	426314	7	NULL	NULL	NULL	NULL	constipation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis and management of constipation and encopresis in childhood .
	manualset3
264505	4	426314	7	NULL	NULL	NULL	NULL	encopresis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis and management of constipation and encopresis in childhood .
	manualset3
264506	5	426314	7	NULL	NULL	NULL	NULL	childhood	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis and management of constipation and encopresis in childhood .
	manualset3
264507	1	426315	7	NULL	NULL	NULL	NULL	Notes 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Notes on the separation of bilirubin by paper chromatography ) .
	manualset3
264508	2	426315	7	NULL	NULL	NULL	NULL	separation 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Notes on the separation of bilirubin by paper chromatography ) .
	manualset3
264509	3	426315	7	NULL	NULL	NULL	NULL	bilirubin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Notes on the separation of bilirubin by paper chromatography ) .
	manualset3
264510	4	426315	7	NULL	NULL	NULL	NULL	paper chromatography	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Notes on the separation of bilirubin by paper chromatography ) .
	manualset3
264511	1	426316	7	NULL	NULL	NULL	NULL	Diagnosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis and management of leiomyosarcoma arising from ovarian vein : Case report and literature review .
	manualset3
264512	2	426316	7	NULL	NULL	NULL	NULL	management 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis and management of leiomyosarcoma arising from ovarian vein : Case report and literature review .
	manualset3
264513	3	426316	7	NULL	NULL	NULL	NULL	leiomyosarcoma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis and management of leiomyosarcoma arising from ovarian vein : Case report and literature review .
	manualset3
264514	4	426316	7	NULL	NULL	NULL	NULL	 ovarian vein	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis and management of leiomyosarcoma arising from ovarian vein : Case report and literature review .
	manualset3
264516	5	426316	7	NULL	NULL	NULL	NULL	Case report 	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis and management of leiomyosarcoma arising from ovarian vein : Case report and literature review .
	manualset3
264517	6	426316	7	NULL	NULL	NULL	NULL	literature review	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis and management of leiomyosarcoma arising from ovarian vein : Case report and literature review .
	manualset3
264520	1	426317	7	NULL	NULL	NULL	NULL	Diagnosis 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis and treatment of thyroid diseases have played a major role in Central European Nuclear Medicine .
	manualset3
264522	2	426317	7	NULL	NULL	NULL	NULL	treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis and treatment of thyroid diseases have played a major role in Central European Nuclear Medicine .
	manualset3
264524	3	426317	7	NULL	NULL	NULL	NULL	thyroid diseases	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis and treatment of thyroid diseases have played a major role in Central European Nuclear Medicine .
	manualset3
264526	4	426317	7	NULL	NULL	NULL	NULL	major role	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis and treatment of thyroid diseases have played a major role in Central European Nuclear Medicine .
	manualset3
264529	5	426317	7	NULL	NULL	NULL	NULL	Central European Nuclear Medicine	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis and treatment of thyroid diseases have played a major role in Central European Nuclear Medicine .
	manualset3
264532	1	426318	7	NULL	NULL	NULL	NULL	Diagnosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis of sarcoidosis by bone marrow trephine biopsy .
	manualset3
264533	2	426318	7	NULL	NULL	NULL	NULL	 sarcoidosis 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis of sarcoidosis by bone marrow trephine biopsy .
	manualset3
264535	3	426318	7	NULL	NULL	NULL	NULL	bone marrow trephine biopsy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis of sarcoidosis by bone marrow trephine biopsy .
	manualset3
264540	1	426319	7	NULL	NULL	NULL	NULL	Diagnosis 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis was made by the radiographic finding of diffuse bilateral lung opacities , and bloody lavage fluid on bronchoscopy .
	manualset3
264543	2	426319	7	NULL	NULL	NULL	NULL	radiographic finding	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis was made by the radiographic finding of diffuse bilateral lung opacities , and bloody lavage fluid on bronchoscopy .
	manualset3
264545	3	426319	7	NULL	NULL	NULL	NULL	 diffuse bilateral lung opacities	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis was made by the radiographic finding of diffuse bilateral lung opacities , and bloody lavage fluid on bronchoscopy .
	manualset3
264547	4	426319	7	NULL	NULL	NULL	NULL	bloody lavage fluid 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis was made by the radiographic finding of diffuse bilateral lung opacities , and bloody lavage fluid on bronchoscopy .
	manualset3
264548	5	426319	7	NULL	NULL	NULL	NULL	bronchoscopy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis was made by the radiographic finding of diffuse bilateral lung opacities , and bloody lavage fluid on bronchoscopy .
	manualset3
264554	1	426320	7	NULL	NULL	NULL	NULL	Diagnosis 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis was performed by superficial lymph node biopsy .
	manualset3
264555	2	426320	7	NULL	NULL	NULL	NULL	superficial lymph node biopsy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnosis was performed by superficial lymph node biopsy .
	manualset3
264556	1	426321	7	NULL	NULL	NULL	NULL	ICU	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Now we need n't rush away from the ICU in Lund ) .
	manualset3
264557	2	426321	7	NULL	NULL	NULL	NULL	 Lund	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Now we need n't rush away from the ICU in Lund ) .
	manualset3
264558	1	426322	7	NULL	NULL	NULL	NULL	Diagnostic accuracy	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic accuracy of self collected vaginal specimens for human papillomavirus compared to clinician collected human papillomavirus specimens : a meta-analysis .
	manualset3
264560	2	426322	7	NULL	NULL	NULL	NULL	self collected vaginal specimens	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic accuracy of self collected vaginal specimens for human papillomavirus compared to clinician collected human papillomavirus specimens : a meta-analysis .
	manualset3
264561	3	426322	7	NULL	NULL	NULL	NULL	 human papillomavirus	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic accuracy of self collected vaginal specimens for human papillomavirus compared to clinician collected human papillomavirus specimens : a meta-analysis .
	manualset3
264564	4	426322	7	NULL	NULL	NULL	NULL	clinician	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic accuracy of self collected vaginal specimens for human papillomavirus compared to clinician collected human papillomavirus specimens : a meta-analysis .
	manualset3
264565	5	426322	7	NULL	NULL	NULL	NULL	human papillomavirus specimens 	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic accuracy of self collected vaginal specimens for human papillomavirus compared to clinician collected human papillomavirus specimens : a meta-analysis .
	manualset3
264567	6	426322	7	NULL	NULL	NULL	NULL	meta-analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic accuracy of self collected vaginal specimens for human papillomavirus compared to clinician collected human papillomavirus specimens : a meta-analysis .
	manualset3
264568	1	426323	7	NULL	NULL	NULL	NULL	Diagnostic value 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic and therapeutic value of laparoscopy for small bowel blunt injuries : A case report .
	manualset3
264569	2	426323	7	NULL	NULL	NULL	NULL	therapeutic value	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic and therapeutic value of laparoscopy for small bowel blunt injuries : A case report .
	manualset3
264570	3	426323	7	NULL	NULL	NULL	NULL	laparoscopy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic and therapeutic value of laparoscopy for small bowel blunt injuries : A case report .
	manualset3
264572	4	426323	7	NULL	NULL	NULL	NULL	small bowel blunt injuries	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic and therapeutic value of laparoscopy for small bowel blunt injuries : A case report .
	manualset3
264573	5	426323	7	NULL	NULL	NULL	NULL	case report	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic and therapeutic value of laparoscopy for small bowel blunt injuries : A case report .
	manualset3
264577	1	426324	7	NULL	NULL	NULL	NULL	Diagnostic approaches	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic approaches incorporate a high clinical index of suspicion , echocardiographic evidence , and inferences about hemodynamic data derived from pulmonary artery catheterization .
	manualset3
264579	2	426324	7	NULL	NULL	NULL	NULL	 high clinical index	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic approaches incorporate a high clinical index of suspicion , echocardiographic evidence , and inferences about hemodynamic data derived from pulmonary artery catheterization .
	manualset3
264581	3	426324	7	NULL	NULL	NULL	NULL	suspicion	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic approaches incorporate a high clinical index of suspicion , echocardiographic evidence , and inferences about hemodynamic data derived from pulmonary artery catheterization .
	manualset3
264583	4	426324	7	NULL	NULL	NULL	NULL	echocardiographic evidence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic approaches incorporate a high clinical index of suspicion , echocardiographic evidence , and inferences about hemodynamic data derived from pulmonary artery catheterization .
	manualset3
264584	5	426324	7	NULL	NULL	NULL	NULL	inferences 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic approaches incorporate a high clinical index of suspicion , echocardiographic evidence , and inferences about hemodynamic data derived from pulmonary artery catheterization .
	manualset3
264586	6	426324	7	NULL	NULL	NULL	NULL	hemodynamic data	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic approaches incorporate a high clinical index of suspicion , echocardiographic evidence , and inferences about hemodynamic data derived from pulmonary artery catheterization .
	manualset3
264589	7	426324	7	NULL	NULL	NULL	NULL	pulmonary artery catheterization	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic approaches incorporate a high clinical index of suspicion , echocardiographic evidence , and inferences about hemodynamic data derived from pulmonary artery catheterization .
	manualset3
264592	1	426325	7	NULL	NULL	NULL	NULL	Diagnostic frequency continuous ultrasonography	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic frequency continuous ultrasonography directly mitigates venular ischemia reperfusion damage .
	manualset3
264593	2	426325	7	NULL	NULL	NULL	NULL	venular ischemia reperfusion damage	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic frequency continuous ultrasonography directly mitigates venular ischemia reperfusion damage .
	manualset3
264595	1	426326	7	NULL	NULL	NULL	NULL	Diagnostic markers	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic markers for ketosis such as acetone and beta-hydroxybutyric acid ( BHBA ) are known , but disease prediction remains an unsolved challenge .
	manualset3
264596	2	426326	7	NULL	NULL	NULL	NULL	 ketosis 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic markers for ketosis such as acetone and beta-hydroxybutyric acid ( BHBA ) are known , but disease prediction remains an unsolved challenge .
	manualset3
264597	3	426326	7	NULL	NULL	NULL	NULL	 acetone	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic markers for ketosis such as acetone and beta-hydroxybutyric acid ( BHBA ) are known , but disease prediction remains an unsolved challenge .
	manualset3
264598	4	426326	7	NULL	NULL	NULL	NULL	 beta-hydroxybutyric acid ( BHBA )	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic markers for ketosis such as acetone and beta-hydroxybutyric acid ( BHBA ) are known , but disease prediction remains an unsolved challenge .
	manualset3
264600	5	426326	7	NULL	NULL	NULL	NULL	disease prediction 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic markers for ketosis such as acetone and beta-hydroxybutyric acid ( BHBA ) are known , but disease prediction remains an unsolved challenge .
	manualset3
264602	6	426326	7	NULL	NULL	NULL	NULL	challenge	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic markers for ketosis such as acetone and beta-hydroxybutyric acid ( BHBA ) are known , but disease prediction remains an unsolved challenge .
	manualset3
264603	1	426327	7	NULL	NULL	NULL	NULL	Diagnostic significance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic significance of the secretin and pancreozymin tests ) .
	manualset3
264605	2	426327	7	NULL	NULL	NULL	NULL	 secretin 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic significance of the secretin and pancreozymin tests ) .
	manualset3
264607	3	426327	7	NULL	NULL	NULL	NULL	 pancreozymin tests	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic significance of the secretin and pancreozymin tests ) .
	manualset3
264609	1	426328	7	NULL	NULL	NULL	NULL	Diagnostic signs 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic signs of cutaneous lymphomas .
	manualset3
264611	2	426328	7	NULL	NULL	NULL	NULL	cutaneous lymphomas	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic signs of cutaneous lymphomas .
	manualset3
264620	1	426329	7	NULL	NULL	NULL	NULL	Diagnostic ultrasound 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic ultrasound assists in determining the size and location of tumors and vital normal structures in patients undergoing radiation therapy .
	manualset3
264621	2	426329	7	NULL	NULL	NULL	NULL	 size	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic ultrasound assists in determining the size and location of tumors and vital normal structures in patients undergoing radiation therapy .
	manualset3
264622	3	426329	7	NULL	NULL	NULL	NULL	location	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic ultrasound assists in determining the size and location of tumors and vital normal structures in patients undergoing radiation therapy .
	manualset3
264626	4	426329	7	NULL	NULL	NULL	NULL	tumors 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic ultrasound assists in determining the size and location of tumors and vital normal structures in patients undergoing radiation therapy .
	manualset3
264627	5	426329	7	NULL	NULL	NULL	NULL	vital normal structures	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic ultrasound assists in determining the size and location of tumors and vital normal structures in patients undergoing radiation therapy .
	manualset3
264629	6	426329	7	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic ultrasound assists in determining the size and location of tumors and vital normal structures in patients undergoing radiation therapy .
	manualset3
264631	7	426329	7	NULL	NULL	NULL	NULL	radiation therapy	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic ultrasound assists in determining the size and location of tumors and vital normal structures in patients undergoing radiation therapy .
	manualset3
264633	1	426330	7	NULL	NULL	NULL	NULL	Nuclear resonance tomography	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Nuclear resonance tomography of the central nervous system ; a good use of the possibilities ) .
	manualset3
264634	2	426330	7	NULL	NULL	NULL	NULL	central nervous system	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Nuclear resonance tomography of the central nervous system ; a good use of the possibilities ) .
	manualset3
264635	3	426330	7	NULL	NULL	NULL	NULL	 good use	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Nuclear resonance tomography of the central nervous system ; a good use of the possibilities ) .
	manualset3
264636	4	426330	7	NULL	NULL	NULL	NULL	possibilities 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Nuclear resonance tomography of the central nervous system ; a good use of the possibilities ) .
	manualset3
246470	1	426331	16	NULL	NULL	0	NULL	Diagnostic work-up	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Diagnostic work-up in patients with diabetes mellitus , in whom gastrointestinal involvement is suspected comprises the assessment of gastrointestinal transit times , endoscopy , esophageal pH-metry or manometry , sonography and lactulose - or glucose-H2-breath tests .
	manualset3
246471	2	426331	16	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Diagnostic work-up in patients with diabetes mellitus , in whom gastrointestinal involvement is suspected comprises the assessment of gastrointestinal transit times , endoscopy , esophageal pH-metry or manometry , sonography and lactulose - or glucose-H2-breath tests .
	manualset3
246472	3	426331	16	NULL	NULL	0	NULL	diabetes mellitus	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Diagnostic work-up in patients with diabetes mellitus , in whom gastrointestinal involvement is suspected comprises the assessment of gastrointestinal transit times , endoscopy , esophageal pH-metry or manometry , sonography and lactulose - or glucose-H2-breath tests .
	manualset3
246473	4	426331	16	NULL	NULL	0	NULL	gastrointestinal involvement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Diagnostic work-up in patients with diabetes mellitus , in whom gastrointestinal involvement is suspected comprises the assessment of gastrointestinal transit times , endoscopy , esophageal pH-metry or manometry , sonography and lactulose - or glucose-H2-breath tests .
	manualset3
246474	5	426331	16	NULL	NULL	0	NULL	assessment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Diagnostic work-up in patients with diabetes mellitus , in whom gastrointestinal involvement is suspected comprises the assessment of gastrointestinal transit times , endoscopy , esophageal pH-metry or manometry , sonography and lactulose - or glucose-H2-breath tests .
	manualset3
246475	6	426331	16	NULL	NULL	NULL	NULL	gastrointestinal transit times	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diagnostic work-up in patients with diabetes mellitus , in whom gastrointestinal involvement is suspected comprises the assessment of gastrointestinal transit times , endoscopy , esophageal pH-metry or manometry , sonography and lactulose - or glucose-H2-breath tests .
	manualset3
246476	7	426331	16	NULL	NULL	0	NULL	endoscopy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Diagnostic work-up in patients with diabetes mellitus , in whom gastrointestinal involvement is suspected comprises the assessment of gastrointestinal transit times , endoscopy , esophageal pH-metry or manometry , sonography and lactulose - or glucose-H2-breath tests .
	manualset3
246477	8	426331	16	NULL	NULL	0	NULL	esophageal pH-metry	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Diagnostic work-up in patients with diabetes mellitus , in whom gastrointestinal involvement is suspected comprises the assessment of gastrointestinal transit times , endoscopy , esophageal pH-metry or manometry , sonography and lactulose - or glucose-H2-breath tests .
	manualset3
246478	9	426331	16	NULL	NULL	0	NULL	manometry	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Diagnostic work-up in patients with diabetes mellitus , in whom gastrointestinal involvement is suspected comprises the assessment of gastrointestinal transit times , endoscopy , esophageal pH-metry or manometry , sonography and lactulose - or glucose-H2-breath tests .
	manualset3
246479	10	426331	16	NULL	NULL	0	NULL	sonography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Diagnostic work-up in patients with diabetes mellitus , in whom gastrointestinal involvement is suspected comprises the assessment of gastrointestinal transit times , endoscopy , esophageal pH-metry or manometry , sonography and lactulose - or glucose-H2-breath tests .
	manualset3
246480	11	426331	16	NULL	NULL	0	NULL	lactulose H2-breath tests	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Diagnostic work-up in patients with diabetes mellitus , in whom gastrointestinal involvement is suspected comprises the assessment of gastrointestinal transit times , endoscopy , esophageal pH-metry or manometry , sonography and lactulose - or glucose-H2-breath tests .
	manualset3
246481	12	426331	16	NULL	NULL	0	NULL	glucose-H2-breath tests	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Diagnostic work-up in patients with diabetes mellitus , in whom gastrointestinal involvement is suspected comprises the assessment of gastrointestinal transit times , endoscopy , esophageal pH-metry or manometry , sonography and lactulose - or glucose-H2-breath tests .
	manualset3
246482	1	426332	16	NULL	NULL	0	NULL	Diameter	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Diameter was determined during application of artificial cerebrospinal fluid containing no drugs and during application of 10 ( -5 ) , 10 ( -4 ) , 10 ( -3 ) , and 10 ( -2 ) M L-arginine ( ARG ) , L-arginine ethyl ester ( AEE ) , N alpha-benzoyl-L-arginine ( NBA ) , N alpha-benzoyl-L-arginine ester ethyl ( BAEE ) , and L-citrulline ( CIT ) .
	manualset3
246483	2	426332	16	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Diameter was determined during application of artificial cerebrospinal fluid containing no drugs and during application of 10 ( -5 ) , 10 ( -4 ) , 10 ( -3 ) , and 10 ( -2 ) M L-arginine ( ARG ) , L-arginine ethyl ester ( AEE ) , N alpha-benzoyl-L-arginine ( NBA ) , N alpha-benzoyl-L-arginine ester ethyl ( BAEE ) , and L-citrulline ( CIT ) .
	manualset3
246484	3	426332	16	NULL	NULL	0	NULL	artificial cerebrospinal fluid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Diameter was determined during application of artificial cerebrospinal fluid containing no drugs and during application of 10 ( -5 ) , 10 ( -4 ) , 10 ( -3 ) , and 10 ( -2 ) M L-arginine ( ARG ) , L-arginine ethyl ester ( AEE ) , N alpha-benzoyl-L-arginine ( NBA ) , N alpha-benzoyl-L-arginine ester ethyl ( BAEE ) , and L-citrulline ( CIT ) .
	manualset3
246485	4	426332	16	NULL	NULL	0	NULL	drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Diameter was determined during application of artificial cerebrospinal fluid containing no drugs and during application of 10 ( -5 ) , 10 ( -4 ) , 10 ( -3 ) , and 10 ( -2 ) M L-arginine ( ARG ) , L-arginine ethyl ester ( AEE ) , N alpha-benzoyl-L-arginine ( NBA ) , N alpha-benzoyl-L-arginine ester ethyl ( BAEE ) , and L-citrulline ( CIT ) .
	manualset3
246486	5	426332	16	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Diameter was determined during application of artificial cerebrospinal fluid containing no drugs and during application of 10 ( -5 ) , 10 ( -4 ) , 10 ( -3 ) , and 10 ( -2 ) M L-arginine ( ARG ) , L-arginine ethyl ester ( AEE ) , N alpha-benzoyl-L-arginine ( NBA ) , N alpha-benzoyl-L-arginine ester ethyl ( BAEE ) , and L-citrulline ( CIT ) .
	manualset3
246487	6	426332	16	NULL	NULL	0	NULL	10 ( -5 ) M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Diameter was determined during application of artificial cerebrospinal fluid containing no drugs and during application of 10 ( -5 ) , 10 ( -4 ) , 10 ( -3 ) , and 10 ( -2 ) M L-arginine ( ARG ) , L-arginine ethyl ester ( AEE ) , N alpha-benzoyl-L-arginine ( NBA ) , N alpha-benzoyl-L-arginine ester ethyl ( BAEE ) , and L-citrulline ( CIT ) .
	manualset3
246488	7	426332	16	NULL	NULL	0	NULL	10 ( -4 ) M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Diameter was determined during application of artificial cerebrospinal fluid containing no drugs and during application of 10 ( -5 ) , 10 ( -4 ) , 10 ( -3 ) , and 10 ( -2 ) M L-arginine ( ARG ) , L-arginine ethyl ester ( AEE ) , N alpha-benzoyl-L-arginine ( NBA ) , N alpha-benzoyl-L-arginine ester ethyl ( BAEE ) , and L-citrulline ( CIT ) .
	manualset3
246489	8	426332	16	NULL	NULL	0	NULL	10 ( -3 ) M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Diameter was determined during application of artificial cerebrospinal fluid containing no drugs and during application of 10 ( -5 ) , 10 ( -4 ) , 10 ( -3 ) , and 10 ( -2 ) M L-arginine ( ARG ) , L-arginine ethyl ester ( AEE ) , N alpha-benzoyl-L-arginine ( NBA ) , N alpha-benzoyl-L-arginine ester ethyl ( BAEE ) , and L-citrulline ( CIT ) .
	manualset3
246490	9	426332	16	NULL	NULL	0	NULL	10 ( -2 ) M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Diameter was determined during application of artificial cerebrospinal fluid containing no drugs and during application of 10 ( -5 ) , 10 ( -4 ) , 10 ( -3 ) , and 10 ( -2 ) M L-arginine ( ARG ) , L-arginine ethyl ester ( AEE ) , N alpha-benzoyl-L-arginine ( NBA ) , N alpha-benzoyl-L-arginine ester ethyl ( BAEE ) , and L-citrulline ( CIT ) .
	manualset3
246495	10	426332	16	NULL	NULL	0	NULL	L-arginine ( ARG )	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Diameter was determined during application of artificial cerebrospinal fluid containing no drugs and during application of 10 ( -5 ) , 10 ( -4 ) , 10 ( -3 ) , and 10 ( -2 ) M L-arginine ( ARG ) , L-arginine ethyl ester ( AEE ) , N alpha-benzoyl-L-arginine ( NBA ) , N alpha-benzoyl-L-arginine ester ethyl ( BAEE ) , and L-citrulline ( CIT ) .
	manualset3
246502	11	426332	16	NULL	NULL	0	NULL	L-arginine ethyl ester ( AEE )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Diameter was determined during application of artificial cerebrospinal fluid containing no drugs and during application of 10 ( -5 ) , 10 ( -4 ) , 10 ( -3 ) , and 10 ( -2 ) M L-arginine ( ARG ) , L-arginine ethyl ester ( AEE ) , N alpha-benzoyl-L-arginine ( NBA ) , N alpha-benzoyl-L-arginine ester ethyl ( BAEE ) , and L-citrulline ( CIT ) .
	manualset3
246524	12	426332	16	NULL	NULL	0	NULL	N alpha-benzoyl-L-arginine ( NBA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Diameter was determined during application of artificial cerebrospinal fluid containing no drugs and during application of 10 ( -5 ) , 10 ( -4 ) , 10 ( -3 ) , and 10 ( -2 ) M L-arginine ( ARG ) , L-arginine ethyl ester ( AEE ) , N alpha-benzoyl-L-arginine ( NBA ) , N alpha-benzoyl-L-arginine ester ethyl ( BAEE ) , and L-citrulline ( CIT ) .
	manualset3
246525	13	426332	16	NULL	NULL	0	NULL	N alpha-benzoyl-L-arginine ester ethyl ( BAEE )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Diameter was determined during application of artificial cerebrospinal fluid containing no drugs and during application of 10 ( -5 ) , 10 ( -4 ) , 10 ( -3 ) , and 10 ( -2 ) M L-arginine ( ARG ) , L-arginine ethyl ester ( AEE ) , N alpha-benzoyl-L-arginine ( NBA ) , N alpha-benzoyl-L-arginine ester ethyl ( BAEE ) , and L-citrulline ( CIT ) .
	manualset3
246531	14	426332	16	NULL	NULL	0	NULL	L-citrulline ( CIT )	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Diameter was determined during application of artificial cerebrospinal fluid containing no drugs and during application of 10 ( -5 ) , 10 ( -4 ) , 10 ( -3 ) , and 10 ( -2 ) M L-arginine ( ARG ) , L-arginine ethyl ester ( AEE ) , N alpha-benzoyl-L-arginine ( NBA ) , N alpha-benzoyl-L-arginine ester ethyl ( BAEE ) , and L-citrulline ( CIT ) .
	manualset3
246536	1	426333	16	NULL	NULL	0	NULL	Dichlorido { 1 - ( N - ( 5-chloro-2-oxidophen-yl ) carboximido-yl ) naphthalen-2-olato-O , N , O ' } ( methanol-O ) tin ( IV )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Dichlorido { 1 - ( N - ( 5-chloro-2-oxidophen-yl ) carboximido-yl ) naphthalen-2-olato-O , N , O ' } ( methanol-O ) tin ( IV ) .
	manualset3
246537	1	426334	16	NULL	NULL	0	NULL	Dichlorodiphenyltrichloroethane serum levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dichlorodiphenyltrichloroethane serum levels and breast cancer risk : a case-control study from Mexico .
	manualset3
246538	2	426334	16	NULL	NULL	0	NULL	breast cancer risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dichlorodiphenyltrichloroethane serum levels and breast cancer risk : a case-control study from Mexico .
	manualset3
246539	3	426334	16	NULL	NULL	0	NULL	case-control study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dichlorodiphenyltrichloroethane serum levels and breast cancer risk : a case-control study from Mexico .
	manualset3
246540	4	426334	16	NULL	NULL	0	NULL	Mexico	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Dichlorodiphenyltrichloroethane serum levels and breast cancer risk : a case-control study from Mexico .
	manualset3
246559	1	426335	16	NULL	NULL	0	NULL	Dichromatic gauging of the spectrum	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dichromatic gauging of the spectrum can not yield unique mixture values for any wavelength because of the large stretches of poor wavelength discrimination .
	manualset3
246579	2	426335	16	NULL	NULL	0	NULL	mixture values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Dichromatic gauging of the spectrum can not yield unique mixture values for any wavelength because of the large stretches of poor wavelength discrimination .
	manualset3
246581	3	426335	16	NULL	NULL	0	NULL	wavelength	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Dichromatic gauging of the spectrum can not yield unique mixture values for any wavelength because of the large stretches of poor wavelength discrimination .
	manualset3
246600	4	426335	16	NULL	NULL	0	NULL	stretches	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Dichromatic gauging of the spectrum can not yield unique mixture values for any wavelength because of the large stretches of poor wavelength discrimination .
	manualset3
246603	5	426335	16	NULL	NULL	NULL	NULL	wavelength discrimination	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dichromatic gauging of the spectrum can not yield unique mixture values for any wavelength because of the large stretches of poor wavelength discrimination .
	manualset3
246605	1	426336	16	NULL	NULL	0	NULL	Dictionaries	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Dictionariesgenerally define pharmacognosy as the subject of the study of crude drugs of plant and animal origin .
	manualset3
246607	2	426336	16	NULL	NULL	0	NULL	pharmacognosy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Dictionariesgenerally define pharmacognosy as the subject of the study of crude drugs of plant and animal origin .
	manualset3
246608	3	426336	16	NULL	NULL	0	NULL	subject	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dictionariesgenerally define pharmacognosy as the subject of the study of crude drugs of plant and animal origin .
	manualset3
246609	4	426336	16	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dictionariesgenerally define pharmacognosy as the subject of the study of crude drugs of plant and animal origin .
	manualset3
246610	5	426336	16	NULL	NULL	NULL	NULL	crude drugs	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dictionariesgenerally define pharmacognosy as the subject of the study of crude drugs of plant and animal origin .
	manualset3
246619	6	426336	16	NULL	NULL	0	NULL	plant origin	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dictionariesgenerally define pharmacognosy as the subject of the study of crude drugs of plant and animal origin .
	manualset3
246620	7	426336	16	NULL	NULL	0	NULL	animal origin	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dictionariesgenerally define pharmacognosy as the subject of the study of crude drugs of plant and animal origin .
	manualset3
246621	1	426337	16	NULL	NULL	0	NULL	Nutritional studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Nutritional and neuropsychiatric studies in chronic iodine deficient girls ( author 's transl ) ) .
	manualset3
246622	2	426337	16	NULL	NULL	0	NULL	neuropsychiatric studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Nutritional and neuropsychiatric studies in chronic iodine deficient girls ( author 's transl ) ) .
	manualset3
246623	3	426337	16	NULL	NULL	0	NULL	chronic iodine deficient girls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Nutritional and neuropsychiatric studies in chronic iodine deficient girls ( author 's transl ) ) .
	manualset3
246624	1	426338	16	NULL	NULL	NULL	NULL	Dietary calcium intake	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dietary calcium and magnesium intake in relation to cancer incidence and mortality in a German prospective cohort ( EPIC-Heidelberg ) .
	manualset3
246625	2	426338	16	NULL	NULL	0	NULL	Dietary magnesium intake	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary calcium and magnesium intake in relation to cancer incidence and mortality in a German prospective cohort ( EPIC-Heidelberg ) .
	manualset3
246626	3	426338	16	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary calcium and magnesium intake in relation to cancer incidence and mortality in a German prospective cohort ( EPIC-Heidelberg ) .
	manualset3
246627	4	426338	16	NULL	NULL	0	NULL	cancer incidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary calcium and magnesium intake in relation to cancer incidence and mortality in a German prospective cohort ( EPIC-Heidelberg ) .
	manualset3
246628	5	426338	16	NULL	NULL	0	NULL	mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary calcium and magnesium intake in relation to cancer incidence and mortality in a German prospective cohort ( EPIC-Heidelberg ) .
	manualset3
246629	6	426338	16	NULL	NULL	0	NULL	German prospective cohort	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary calcium and magnesium intake in relation to cancer incidence and mortality in a German prospective cohort ( EPIC-Heidelberg ) .
	manualset3
246638	7	426338	16	NULL	NULL	0	NULL	EPIC	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary calcium and magnesium intake in relation to cancer incidence and mortality in a German prospective cohort ( EPIC-Heidelberg ) .
	manualset3
246639	8	426338	16	NULL	NULL	0	NULL	Heidelberg	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary calcium and magnesium intake in relation to cancer incidence and mortality in a German prospective cohort ( EPIC-Heidelberg ) .
	manualset3
246660	1	426339	16	NULL	NULL	0	NULL	Dietary carotenoids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary carotenoids have been thought to have beneficial effects on human health through their antioxidant activity , provitamin A activity , and effects on cancer cell propagation .
	manualset3
246665	2	426339	16	NULL	NULL	0	NULL	effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary carotenoids have been thought to have beneficial effects on human health through their antioxidant activity , provitamin A activity , and effects on cancer cell propagation .
	manualset3
246670	3	426339	16	NULL	NULL	0	NULL	health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary carotenoids have been thought to have beneficial effects on human health through their antioxidant activity , provitamin A activity , and effects on cancer cell propagation .
	manualset3
246671	4	426339	16	NULL	NULL	0	NULL	antioxidant activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary carotenoids have been thought to have beneficial effects on human health through their antioxidant activity , provitamin A activity , and effects on cancer cell propagation .
	manualset3
246672	5	426339	16	NULL	NULL	0	NULL	provitamin A activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary carotenoids have been thought to have beneficial effects on human health through their antioxidant activity , provitamin A activity , and effects on cancer cell propagation .
	manualset3
246673	6	426339	16	NULL	NULL	0	NULL	effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary carotenoids have been thought to have beneficial effects on human health through their antioxidant activity , provitamin A activity , and effects on cancer cell propagation .
	manualset3
246675	7	426339	16	NULL	NULL	NULL	NULL	cancer cell propagation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dietary carotenoids have been thought to have beneficial effects on human health through their antioxidant activity , provitamin A activity , and effects on cancer cell propagation .
	manualset3
246681	1	426340	16	NULL	NULL	NULL	NULL	Dietary fructose	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dietary fructose effects on lipoprotein metabolism and risk for coronary artery disease .
	manualset3
246683	2	426340	16	NULL	NULL	0	NULL	effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary fructose effects on lipoprotein metabolism and risk for coronary artery disease .
	manualset3
246684	3	426340	16	NULL	NULL	0	NULL	lipoprotein metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary fructose effects on lipoprotein metabolism and risk for coronary artery disease .
	manualset3
246685	4	426340	16	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary fructose effects on lipoprotein metabolism and risk for coronary artery disease .
	manualset3
246686	5	426340	16	NULL	NULL	0	NULL	coronary artery disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary fructose effects on lipoprotein metabolism and risk for coronary artery disease .
	manualset3
246552	1	426341	16	NULL	NULL	0	NULL	Dietary interventions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary interventions are effective ways to extend or shorten lifespan .
	manualset3
246553	2	426341	16	NULL	NULL	0	NULL	ways	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary interventions are effective ways to extend or shorten lifespan .
	manualset3
246554	3	426341	16	NULL	NULL	0	NULL	lifespan	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary interventions are effective ways to extend or shorten lifespan .
	manualset3
246570	1	426342	16	NULL	NULL	0	NULL	Dietary n-6 polyunsaturated fatty acid ( PUFA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary n-6 polyunsaturated fatty acid ( PUFA ) deprivation in rodents reduces brain arachidonic acid ( 20 : 4 n-6 ) concentration and 20 : 4 n-6-preferring cytosolic phospholipase A ( 2 ) ( cPLA ( 2 ) - IVA ) and cyclooxygenase ( COX ) -2 expression , while increasing brain docosahexaenoic acid ( DHA , 22 : 6 n-3 ) concentration and DHA-selective calcium-independent phospholipase A ( 2 ) ( iPLA ( 2 ) ) - VIA expression .
	manualset3
246571	2	426342	16	NULL	NULL	NULL	NULL	deprivation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dietary n-6 polyunsaturated fatty acid ( PUFA ) deprivation in rodents reduces brain arachidonic acid ( 20 : 4 n-6 ) concentration and 20 : 4 n-6-preferring cytosolic phospholipase A ( 2 ) ( cPLA ( 2 ) - IVA ) and cyclooxygenase ( COX ) -2 expression , while increasing brain docosahexaenoic acid ( DHA , 22 : 6 n-3 ) concentration and DHA-selective calcium-independent phospholipase A ( 2 ) ( iPLA ( 2 ) ) - VIA expression .
	manualset3
246572	3	426342	16	NULL	NULL	0	NULL	 rodents	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary n-6 polyunsaturated fatty acid ( PUFA ) deprivation in rodents reduces brain arachidonic acid ( 20 : 4 n-6 ) concentration and 20 : 4 n-6-preferring cytosolic phospholipase A ( 2 ) ( cPLA ( 2 ) - IVA ) and cyclooxygenase ( COX ) -2 expression , while increasing brain docosahexaenoic acid ( DHA , 22 : 6 n-3 ) concentration and DHA-selective calcium-independent phospholipase A ( 2 ) ( iPLA ( 2 ) ) - VIA expression .
	manualset3
246577	4	426342	16	NULL	NULL	NULL	NULL	brain arachidonic acid ( 20 : 4 n-6 ) concentration 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dietary n-6 polyunsaturated fatty acid ( PUFA ) deprivation in rodents reduces brain arachidonic acid ( 20 : 4 n-6 ) concentration and 20 : 4 n-6-preferring cytosolic phospholipase A ( 2 ) ( cPLA ( 2 ) - IVA ) and cyclooxygenase ( COX ) -2 expression , while increasing brain docosahexaenoic acid ( DHA , 22 : 6 n-3 ) concentration and DHA-selective calcium-independent phospholipase A ( 2 ) ( iPLA ( 2 ) ) - VIA expression .
	manualset3
246587	5	426342	16	NULL	NULL	0	NULL	20 : 4 n-6	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary n-6 polyunsaturated fatty acid ( PUFA ) deprivation in rodents reduces brain arachidonic acid ( 20 : 4 n-6 ) concentration and 20 : 4 n-6-preferring cytosolic phospholipase A ( 2 ) ( cPLA ( 2 ) - IVA ) and cyclooxygenase ( COX ) -2 expression , while increasing brain docosahexaenoic acid ( DHA , 22 : 6 n-3 ) concentration and DHA-selective calcium-independent phospholipase A ( 2 ) ( iPLA ( 2 ) ) - VIA expression .
	manualset3
246588	6	426342	16	NULL	NULL	NULL	NULL	cytosolic phospholipase A ( 2 ) ( cPLA ( 2 ) - IVA ) expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dietary n-6 polyunsaturated fatty acid ( PUFA ) deprivation in rodents reduces brain arachidonic acid ( 20 : 4 n-6 ) concentration and 20 : 4 n-6-preferring cytosolic phospholipase A ( 2 ) ( cPLA ( 2 ) - IVA ) and cyclooxygenase ( COX ) -2 expression , while increasing brain docosahexaenoic acid ( DHA , 22 : 6 n-3 ) concentration and DHA-selective calcium-independent phospholipase A ( 2 ) ( iPLA ( 2 ) ) - VIA expression .
	manualset3
246590	7	426342	16	NULL	NULL	0	NULL	cyclooxygenase ( COX ) -2 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary n-6 polyunsaturated fatty acid ( PUFA ) deprivation in rodents reduces brain arachidonic acid ( 20 : 4 n-6 ) concentration and 20 : 4 n-6-preferring cytosolic phospholipase A ( 2 ) ( cPLA ( 2 ) - IVA ) and cyclooxygenase ( COX ) -2 expression , while increasing brain docosahexaenoic acid ( DHA , 22 : 6 n-3 ) concentration and DHA-selective calcium-independent phospholipase A ( 2 ) ( iPLA ( 2 ) ) - VIA expression .
	manualset3
246591	8	426342	16	NULL	NULL	NULL	NULL	brain docosahexaenoic acid ( DHA , 22 : 6 n-3 ) concentration	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dietary n-6 polyunsaturated fatty acid ( PUFA ) deprivation in rodents reduces brain arachidonic acid ( 20 : 4 n-6 ) concentration and 20 : 4 n-6-preferring cytosolic phospholipase A ( 2 ) ( cPLA ( 2 ) - IVA ) and cyclooxygenase ( COX ) -2 expression , while increasing brain docosahexaenoic acid ( DHA , 22 : 6 n-3 ) concentration and DHA-selective calcium-independent phospholipase A ( 2 ) ( iPLA ( 2 ) ) - VIA expression .
	manualset3
246594	9	426342	16	NULL	NULL	0	NULL	DHA-selective calcium-independent phospholipase A ( 2 ) ( iPLA ( 2 ) ) - VIA expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary n-6 polyunsaturated fatty acid ( PUFA ) deprivation in rodents reduces brain arachidonic acid ( 20 : 4 n-6 ) concentration and 20 : 4 n-6-preferring cytosolic phospholipase A ( 2 ) ( cPLA ( 2 ) - IVA ) and cyclooxygenase ( COX ) -2 expression , while increasing brain docosahexaenoic acid ( DHA , 22 : 6 n-3 ) concentration and DHA-selective calcium-independent phospholipase A ( 2 ) ( iPLA ( 2 ) ) - VIA expression .
	manualset3
246599	1	426343	16	NULL	NULL	NULL	NULL	Dietary omega-3 fatty acids	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dietary omega-3 fatty acids partially correct the enhanced in vivo uptake of glucose in diabetic rats .
	manualset3
246601	2	426343	16	NULL	NULL	NULL	NULL	uptake of glucose	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dietary omega-3 fatty acids partially correct the enhanced in vivo uptake of glucose in diabetic rats .
	manualset3
246606	4	426343	16	NULL	NULL	0	NULL	diabetic rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary omega-3 fatty acids partially correct the enhanced in vivo uptake of glucose in diabetic rats .
	manualset3
246612	1	426344	16	NULL	NULL	0	NULL	Dietary plasma protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary plasma protein reduces small intestinal growth and lamina propria cell density in early weaned pigs .
	manualset3
246613	2	426344	16	NULL	NULL	0	NULL	small intestinal growth	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary plasma protein reduces small intestinal growth and lamina propria cell density in early weaned pigs .
	manualset3
246614	3	426344	16	NULL	NULL	NULL	NULL	lamina propria cell density	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dietary plasma protein reduces small intestinal growth and lamina propria cell density in early weaned pigs .
	manualset3
246616	5	426344	16	NULL	NULL	0	NULL	weaned pigs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary plasma protein reduces small intestinal growth and lamina propria cell density in early weaned pigs .
	manualset3
246655	1	426345	16	NULL	NULL	0	NULL	Dietary protein restriction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary protein restriction , progressive loss of renal adaptive capacity , and uremic toxicity may contribute to the development of malnutrition and water retention in severe chronic renal failure ( CRF ) .
	manualset3
246659	2	426345	16	NULL	NULL	NULL	NULL	progressive loss	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dietary protein restriction , progressive loss of renal adaptive capacity , and uremic toxicity may contribute to the development of malnutrition and water retention in severe chronic renal failure ( CRF ) .
	manualset3
246661	3	426345	16	NULL	NULL	0	NULL	renal adaptive capacity 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary protein restriction , progressive loss of renal adaptive capacity , and uremic toxicity may contribute to the development of malnutrition and water retention in severe chronic renal failure ( CRF ) .
	manualset3
246664	4	426345	16	NULL	NULL	0	NULL	uremic toxicity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary protein restriction , progressive loss of renal adaptive capacity , and uremic toxicity may contribute to the development of malnutrition and water retention in severe chronic renal failure ( CRF ) .
	manualset3
246669	5	426345	16	NULL	NULL	0	NULL	malnutrition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary protein restriction , progressive loss of renal adaptive capacity , and uremic toxicity may contribute to the development of malnutrition and water retention in severe chronic renal failure ( CRF ) .
	manualset3
246674	6	426345	16	NULL	NULL	0	NULL	water retention	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary protein restriction , progressive loss of renal adaptive capacity , and uremic toxicity may contribute to the development of malnutrition and water retention in severe chronic renal failure ( CRF ) .
	manualset3
246676	7	426345	16	NULL	NULL	0	NULL	severe chronic renal failure ( CRF )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary protein restriction , progressive loss of renal adaptive capacity , and uremic toxicity may contribute to the development of malnutrition and water retention in severe chronic renal failure ( CRF ) .
	manualset3
246687	1	426346	16	NULL	NULL	NULL	NULL	Dietary repair	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dietary repair of defective lipogenesis and cholesterogenesis ( from C14-acetate ) in the liver of the hypophysectomized rat .
	manualset3
246688	2	426346	16	NULL	NULL	NULL	NULL	lipogenesis 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dietary repair of defective lipogenesis and cholesterogenesis ( from C14-acetate ) in the liver of the hypophysectomized rat .
	manualset3
246705	3	426346	16	NULL	NULL	NULL	NULL	cholesterogenesis	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dietary repair of defective lipogenesis and cholesterogenesis ( from C14-acetate ) in the liver of the hypophysectomized rat .
	manualset3
246706	4	426346	16	NULL	NULL	0	NULL	C14-acetate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary repair of defective lipogenesis and cholesterogenesis ( from C14-acetate ) in the liver of the hypophysectomized rat .
	manualset3
246714	5	426346	16	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary repair of defective lipogenesis and cholesterogenesis ( from C14-acetate ) in the liver of the hypophysectomized rat .
	manualset3
246715	6	426346	16	NULL	NULL	0	NULL	hypophysectomized rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary repair of defective lipogenesis and cholesterogenesis ( from C14-acetate ) in the liver of the hypophysectomized rat .
	manualset3
246726	1	426347	16	NULL	NULL	0	NULL	Dietary strategies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary strategies for successful weight loss and maintenance : more evidence required .
	manualset3
246731	2	426347	16	NULL	NULL	0	NULL	weight loss	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary strategies for successful weight loss and maintenance : more evidence required .
	manualset3
246743	3	426347	16	NULL	NULL	0	NULL	maintenance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary strategies for successful weight loss and maintenance : more evidence required .
	manualset3
246747	4	426347	16	NULL	NULL	NULL	NULL	evidence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dietary strategies for successful weight loss and maintenance : more evidence required .
	manualset3
246758	1	426348	16	NULL	NULL	NULL	NULL	Dietary supplementation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dietary supplementation with L-methionine impairs the utilization of urea-nitrogen and increases 5-L-oxoprolinuria in normal women consuming a low protein diet .
	manualset3
246762	2	426348	16	NULL	NULL	0	NULL	L-methionine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary supplementation with L-methionine impairs the utilization of urea-nitrogen and increases 5-L-oxoprolinuria in normal women consuming a low protein diet .
	manualset3
246768	3	426348	16	NULL	NULL	0	NULL	utilization of urea-nitrogen	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary supplementation with L-methionine impairs the utilization of urea-nitrogen and increases 5-L-oxoprolinuria in normal women consuming a low protein diet .
	manualset3
246773	4	426348	16	NULL	NULL	0	NULL	 increases 5-L-oxoprolinuria	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary supplementation with L-methionine impairs the utilization of urea-nitrogen and increases 5-L-oxoprolinuria in normal women consuming a low protein diet .
	manualset3
246780	5	426348	16	NULL	NULL	0	NULL	normal women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary supplementation with L-methionine impairs the utilization of urea-nitrogen and increases 5-L-oxoprolinuria in normal women consuming a low protein diet .
	manualset3
246787	6	426348	16	NULL	NULL	0	NULL	low protein diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary supplementation with L-methionine impairs the utilization of urea-nitrogen and increases 5-L-oxoprolinuria in normal women consuming a low protein diet .
	manualset3
246816	1	426349	16	NULL	NULL	0	NULL	Dietary therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary therapy is helpful , but many patients continue to have significant dyslipoproteinemia after both dietary modification and fish oil supplementation .
	manualset3
246835	2	426349	16	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary therapy is helpful , but many patients continue to have significant dyslipoproteinemia after both dietary modification and fish oil supplementation .
	manualset3
246838	3	426349	16	NULL	NULL	0	NULL	dyslipoproteinemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary therapy is helpful , but many patients continue to have significant dyslipoproteinemia after both dietary modification and fish oil supplementation .
	manualset3
246841	4	426349	16	NULL	NULL	NULL	NULL	dietary modification	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dietary therapy is helpful , but many patients continue to have significant dyslipoproteinemia after both dietary modification and fish oil supplementation .
	manualset3
246842	5	426349	16	NULL	NULL	NULL	NULL	fish oil supplementation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dietary therapy is helpful , but many patients continue to have significant dyslipoproteinemia after both dietary modification and fish oil supplementation .
	manualset3
246855	1	426350	16	NULL	NULL	0	NULL	Dietary vegetable oil	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary vegetable oil and wood derived plant stanol esters reduce atherosclerotic lesion size and severity in apoE * 3-Leiden transgenic mice .
	manualset3
246888	2	426350	16	NULL	NULL	0	NULL	wood	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary vegetable oil and wood derived plant stanol esters reduce atherosclerotic lesion size and severity in apoE * 3-Leiden transgenic mice .
	manualset3
246890	3	426350	16	NULL	NULL	0	NULL	plant stanol esters	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary vegetable oil and wood derived plant stanol esters reduce atherosclerotic lesion size and severity in apoE * 3-Leiden transgenic mice .
	manualset3
246894	4	426350	16	NULL	NULL	NULL	NULL	atherosclerotic lesion size 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dietary vegetable oil and wood derived plant stanol esters reduce atherosclerotic lesion size and severity in apoE * 3-Leiden transgenic mice .
	manualset3
246895	5	426350	16	NULL	NULL	0	NULL	atherosclerotic lesion severity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary vegetable oil and wood derived plant stanol esters reduce atherosclerotic lesion size and severity in apoE * 3-Leiden transgenic mice .
	manualset3
246896	6	426350	16	NULL	NULL	0	NULL	apoE * 3-Leiden transgenic mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Dietary vegetable oil and wood derived plant stanol esters reduce atherosclerotic lesion size and severity in apoE * 3-Leiden transgenic mice .
	manualset3
246712	1	426351	16	NULL	NULL	0	NULL	Dieting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Dieting decreases plasma tryptophan and increases the prolactin response to d-fenfluramine in women but not men .
	manualset3
246718	2	426351	16	NULL	NULL	0	NULL	plasma tryptophan	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Dieting decreases plasma tryptophan and increases the prolactin response to d-fenfluramine in women but not men .
	manualset3
246722	3	426351	16	NULL	NULL	NULL	NULL	prolactin response	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dieting decreases plasma tryptophan and increases the prolactin response to d-fenfluramine in women but not men .
	manualset3
246732	4	426351	16	NULL	NULL	0	NULL	d-fenfluramine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Dieting decreases plasma tryptophan and increases the prolactin response to d-fenfluramine in women but not men .
	manualset3
246734	5	426351	16	NULL	NULL	0	NULL	women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Dieting decreases plasma tryptophan and increases the prolactin response to d-fenfluramine in women but not men .
	manualset3
246736	6	426351	16	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Dieting decreases plasma tryptophan and increases the prolactin response to d-fenfluramine in women but not men .
	manualset3
246738	1	426352	16	NULL	NULL	0	NULL	Diets	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Diets were supplemented with 0.33 % of cholesterol and differed in the content of pectin ( three levels ) and of phytosterols ( three levels ) .
	manualset3
246740	2	426352	16	NULL	NULL	0	NULL	0.33 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Diets were supplemented with 0.33 % of cholesterol and differed in the content of pectin ( three levels ) and of phytosterols ( three levels ) .
	manualset3
246742	3	426352	16	NULL	NULL	0	NULL	cholesterol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Diets were supplemented with 0.33 % of cholesterol and differed in the content of pectin ( three levels ) and of phytosterols ( three levels ) .
	manualset3
246751	4	426352	16	NULL	NULL	0	NULL	pectin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Diets were supplemented with 0.33 % of cholesterol and differed in the content of pectin ( three levels ) and of phytosterols ( three levels ) .
	manualset3
246752	5	426352	16	NULL	NULL	0	NULL	three levels 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Diets were supplemented with 0.33 % of cholesterol and differed in the content of pectin ( three levels ) and of phytosterols ( three levels ) .
	manualset3
246753	6	426352	16	NULL	NULL	0	NULL	phytosterols	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Diets were supplemented with 0.33 % of cholesterol and differed in the content of pectin ( three levels ) and of phytosterols ( three levels ) .
	manualset3
246754	7	426352	16	NULL	NULL	0	NULL	three levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Diets were supplemented with 0.33 % of cholesterol and differed in the content of pectin ( three levels ) and of phytosterols ( three levels ) .
	manualset3
246757	1	426353	16	NULL	NULL	0	NULL	Difference spectra	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Difference spectra revealed the presence of cytochromes ( a + a3 ) , b and c. Respiratory control was stimulated 2-fold by ADP with different exogenous oxidizable substrates .
	manualset3
246761	2	426353	16	NULL	NULL	NULL	NULL	presence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Difference spectra revealed the presence of cytochromes ( a + a3 ) , b and c. Respiratory control was stimulated 2-fold by ADP with different exogenous oxidizable substrates .
	manualset3
246766	3	426353	16	NULL	NULL	NULL	NULL	cytochromes ( a + a3 )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Difference spectra revealed the presence of cytochromes ( a + a3 ) , b and c. Respiratory control was stimulated 2-fold by ADP with different exogenous oxidizable substrates .
	manualset3
246790	4	426353	16	NULL	NULL	0	NULL	cytochromes b	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Difference spectra revealed the presence of cytochromes ( a + a3 ) , b and c. Respiratory control was stimulated 2-fold by ADP with different exogenous oxidizable substrates .
	manualset3
246792	5	426353	16	NULL	NULL	0	NULL	cytochrome c	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Difference spectra revealed the presence of cytochromes ( a + a3 ) , b and c. Respiratory control was stimulated 2-fold by ADP with different exogenous oxidizable substrates .
	manualset3
246794	6	426353	16	NULL	NULL	NULL	NULL	Respiratory control	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Difference spectra revealed the presence of cytochromes ( a + a3 ) , b and c. Respiratory control was stimulated 2-fold by ADP with different exogenous oxidizable substrates .
	manualset3
246795	7	426353	16	NULL	NULL	0	NULL	2-fold	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Difference spectra revealed the presence of cytochromes ( a + a3 ) , b and c. Respiratory control was stimulated 2-fold by ADP with different exogenous oxidizable substrates .
	manualset3
246796	8	426353	16	NULL	NULL	0	NULL	ADP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Difference spectra revealed the presence of cytochromes ( a + a3 ) , b and c. Respiratory control was stimulated 2-fold by ADP with different exogenous oxidizable substrates .
	manualset3
246797	9	426353	16	NULL	NULL	0	NULL	oxidizable substrates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Difference spectra revealed the presence of cytochromes ( a + a3 ) , b and c. Respiratory control was stimulated 2-fold by ADP with different exogenous oxidizable substrates .
	manualset3
246803	1	426354	16	NULL	NULL	0	NULL	OBSERVATIONS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( OBSERVATIONS ON URINARY CATECHOLAMINES IN AGED SUBJECTS TREATED WITH NIALAMIDE ) .
	manualset3
246805	2	426354	16	NULL	NULL	NULL	NULL	URINARY CATECHOLAMINES	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( OBSERVATIONS ON URINARY CATECHOLAMINES IN AGED SUBJECTS TREATED WITH NIALAMIDE ) .
	manualset3
246806	3	426354	16	NULL	NULL	0	NULL	AGED SUBJECTS	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( OBSERVATIONS ON URINARY CATECHOLAMINES IN AGED SUBJECTS TREATED WITH NIALAMIDE ) .
	manualset3
246808	4	426354	16	NULL	NULL	0	NULL	NIALAMIDE	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( OBSERVATIONS ON URINARY CATECHOLAMINES IN AGED SUBJECTS TREATED WITH NIALAMIDE ) .
	manualset3
246818	1	426355	16	NULL	NULL	0	NULL	Differences	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences between clones were apparent in sapwood but not in bark and were due to peaks in the aliphatic and carbohydrate regions .
	manualset3
246820	2	426355	16	NULL	NULL	0	NULL	clones	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences between clones were apparent in sapwood but not in bark and were due to peaks in the aliphatic and carbohydrate regions .
	manualset3
246827	3	426355	16	NULL	NULL	0	NULL	sapwood	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences between clones were apparent in sapwood but not in bark and were due to peaks in the aliphatic and carbohydrate regions .
	manualset3
246829	4	426355	16	NULL	NULL	0	NULL	bark	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences between clones were apparent in sapwood but not in bark and were due to peaks in the aliphatic and carbohydrate regions .
	manualset3
246831	5	426355	16	NULL	NULL	0	NULL	peaks	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences between clones were apparent in sapwood but not in bark and were due to peaks in the aliphatic and carbohydrate regions .
	manualset3
246834	6	426355	16	NULL	NULL	0	NULL	aliphatic regions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences between clones were apparent in sapwood but not in bark and were due to peaks in the aliphatic and carbohydrate regions .
	manualset3
246836	7	426355	16	NULL	NULL	0	NULL	carbohydrate regions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences between clones were apparent in sapwood but not in bark and were due to peaks in the aliphatic and carbohydrate regions .
	manualset3
246837	1	426356	16	NULL	NULL	NULL	NULL	Differences	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differences between the three rSMC populations were observed with regard to proliferative activity and gene expression patterns , suggesting the retention of some tissue-specific cell characteristics .
	manualset3
246839	2	426356	16	NULL	NULL	NULL	NULL	three	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differences between the three rSMC populations were observed with regard to proliferative activity and gene expression patterns , suggesting the retention of some tissue-specific cell characteristics .
	manualset3
246840	3	426356	16	NULL	NULL	0	NULL	rSMC populations	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences between the three rSMC populations were observed with regard to proliferative activity and gene expression patterns , suggesting the retention of some tissue-specific cell characteristics .
	manualset3
246844	4	426356	16	NULL	NULL	0	NULL	regard	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences between the three rSMC populations were observed with regard to proliferative activity and gene expression patterns , suggesting the retention of some tissue-specific cell characteristics .
	manualset3
246846	5	426356	16	NULL	NULL	0	NULL	proliferative activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences between the three rSMC populations were observed with regard to proliferative activity and gene expression patterns , suggesting the retention of some tissue-specific cell characteristics .
	manualset3
246847	6	426356	16	NULL	NULL	NULL	NULL	gene expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differences between the three rSMC populations were observed with regard to proliferative activity and gene expression patterns , suggesting the retention of some tissue-specific cell characteristics .
	manualset3
246850	7	426356	16	NULL	NULL	0	NULL	patterns	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences between the three rSMC populations were observed with regard to proliferative activity and gene expression patterns , suggesting the retention of some tissue-specific cell characteristics .
	manualset3
246852	8	426356	16	NULL	NULL	NULL	NULL	retention	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differences between the three rSMC populations were observed with regard to proliferative activity and gene expression patterns , suggesting the retention of some tissue-specific cell characteristics .
	manualset3
246859	9	426356	16	NULL	NULL	0	NULL	tissue-specific cell characteristics	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences between the three rSMC populations were observed with regard to proliferative activity and gene expression patterns , suggesting the retention of some tissue-specific cell characteristics .
	manualset3
246862	1	426357	16	NULL	NULL	0	NULL	Differences	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in MDMA pharmacokinetics between baboons and humans suggest that the baboon may not be ideal for modeling human MDMA exposure .
	manualset3
246866	2	426357	16	NULL	NULL	0	NULL	MDMA	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in MDMA pharmacokinetics between baboons and humans suggest that the baboon may not be ideal for modeling human MDMA exposure .
	manualset3
246867	3	426357	16	NULL	NULL	NULL	NULL	pharmacokinetics	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differences in MDMA pharmacokinetics between baboons and humans suggest that the baboon may not be ideal for modeling human MDMA exposure .
	manualset3
246868	4	426357	16	NULL	NULL	0	NULL	baboons	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in MDMA pharmacokinetics between baboons and humans suggest that the baboon may not be ideal for modeling human MDMA exposure .
	manualset3
246869	5	426357	16	NULL	NULL	0	NULL	humans	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in MDMA pharmacokinetics between baboons and humans suggest that the baboon may not be ideal for modeling human MDMA exposure .
	manualset3
246875	6	426357	16	NULL	NULL	0	NULL	baboon	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in MDMA pharmacokinetics between baboons and humans suggest that the baboon may not be ideal for modeling human MDMA exposure .
	manualset3
246878	7	426357	16	NULL	NULL	0	NULL	human	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in MDMA pharmacokinetics between baboons and humans suggest that the baboon may not be ideal for modeling human MDMA exposure .
	manualset3
246880	8	426357	16	NULL	NULL	0	NULL	MDMA	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in MDMA pharmacokinetics between baboons and humans suggest that the baboon may not be ideal for modeling human MDMA exposure .
	manualset3
246882	9	426357	16	NULL	NULL	0	NULL	exposure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in MDMA pharmacokinetics between baboons and humans suggest that the baboon may not be ideal for modeling human MDMA exposure .
	manualset3
246889	1	426358	16	NULL	NULL	0	NULL	Differences	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in TRAIL-induced changes of Mcl-1 expression among distinct human colon epithelial cell lines .
	manualset3
246891	2	426358	16	NULL	NULL	NULL	NULL	TRAIL-induced changes	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differences in TRAIL-induced changes of Mcl-1 expression among distinct human colon epithelial cell lines .
	manualset3
246892	3	426358	16	NULL	NULL	0	NULL	Mcl-1 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in TRAIL-induced changes of Mcl-1 expression among distinct human colon epithelial cell lines .
	manualset3
246893	4	426358	16	NULL	NULL	0	NULL	human colon epithelial cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in TRAIL-induced changes of Mcl-1 expression among distinct human colon epithelial cell lines .
	manualset3
246897	1	426359	16	NULL	NULL	0	NULL	Differences	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in gene stoichiometry in the Global Ocean Survey metagenomic data set compared with 39 sequenced isolates indicated that natural Roseobacter populations differ systematically in several genomic attributes from their cultured representatives , including fewer genes for signal transduction and cell surface modifications but more genes for Sec-like protein secretion systems , anaplerotic CO ( 2 ) incorporation , and phosphorus and sulfate uptake .
	manualset3
246898	2	426359	16	NULL	NULL	0	NULL	gene stoichiometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in gene stoichiometry in the Global Ocean Survey metagenomic data set compared with 39 sequenced isolates indicated that natural Roseobacter populations differ systematically in several genomic attributes from their cultured representatives , including fewer genes for signal transduction and cell surface modifications but more genes for Sec-like protein secretion systems , anaplerotic CO ( 2 ) incorporation , and phosphorus and sulfate uptake .
	manualset3
246899	3	426359	16	NULL	NULL	0	NULL	Global Ocean Survey metagenomic data set	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in gene stoichiometry in the Global Ocean Survey metagenomic data set compared with 39 sequenced isolates indicated that natural Roseobacter populations differ systematically in several genomic attributes from their cultured representatives , including fewer genes for signal transduction and cell surface modifications but more genes for Sec-like protein secretion systems , anaplerotic CO ( 2 ) incorporation , and phosphorus and sulfate uptake .
	manualset3
246900	4	426359	16	NULL	NULL	0	NULL	39	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in gene stoichiometry in the Global Ocean Survey metagenomic data set compared with 39 sequenced isolates indicated that natural Roseobacter populations differ systematically in several genomic attributes from their cultured representatives , including fewer genes for signal transduction and cell surface modifications but more genes for Sec-like protein secretion systems , anaplerotic CO ( 2 ) incorporation , and phosphorus and sulfate uptake .
	manualset3
246901	5	426359	16	NULL	NULL	0	NULL	sequenced isolates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in gene stoichiometry in the Global Ocean Survey metagenomic data set compared with 39 sequenced isolates indicated that natural Roseobacter populations differ systematically in several genomic attributes from their cultured representatives , including fewer genes for signal transduction and cell surface modifications but more genes for Sec-like protein secretion systems , anaplerotic CO ( 2 ) incorporation , and phosphorus and sulfate uptake .
	manualset3
246902	6	426359	16	NULL	NULL	0	NULL	Roseobacter populations	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in gene stoichiometry in the Global Ocean Survey metagenomic data set compared with 39 sequenced isolates indicated that natural Roseobacter populations differ systematically in several genomic attributes from their cultured representatives , including fewer genes for signal transduction and cell surface modifications but more genes for Sec-like protein secretion systems , anaplerotic CO ( 2 ) incorporation , and phosphorus and sulfate uptake .
	manualset3
246903	7	426359	16	NULL	NULL	0	NULL	genomic attributes	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in gene stoichiometry in the Global Ocean Survey metagenomic data set compared with 39 sequenced isolates indicated that natural Roseobacter populations differ systematically in several genomic attributes from their cultured representatives , including fewer genes for signal transduction and cell surface modifications but more genes for Sec-like protein secretion systems , anaplerotic CO ( 2 ) incorporation , and phosphorus and sulfate uptake .
	manualset3
246904	8	426359	16	NULL	NULL	0	NULL	cultured representatives	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in gene stoichiometry in the Global Ocean Survey metagenomic data set compared with 39 sequenced isolates indicated that natural Roseobacter populations differ systematically in several genomic attributes from their cultured representatives , including fewer genes for signal transduction and cell surface modifications but more genes for Sec-like protein secretion systems , anaplerotic CO ( 2 ) incorporation , and phosphorus and sulfate uptake .
	manualset3
246905	9	426359	16	NULL	NULL	0	NULL	genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in gene stoichiometry in the Global Ocean Survey metagenomic data set compared with 39 sequenced isolates indicated that natural Roseobacter populations differ systematically in several genomic attributes from their cultured representatives , including fewer genes for signal transduction and cell surface modifications but more genes for Sec-like protein secretion systems , anaplerotic CO ( 2 ) incorporation , and phosphorus and sulfate uptake .
	manualset3
246906	10	426359	16	NULL	NULL	NULL	NULL	signal transduction	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differences in gene stoichiometry in the Global Ocean Survey metagenomic data set compared with 39 sequenced isolates indicated that natural Roseobacter populations differ systematically in several genomic attributes from their cultured representatives , including fewer genes for signal transduction and cell surface modifications but more genes for Sec-like protein secretion systems , anaplerotic CO ( 2 ) incorporation , and phosphorus and sulfate uptake .
	manualset3
246907	11	426359	16	NULL	NULL	NULL	NULL	cell surface modifications	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differences in gene stoichiometry in the Global Ocean Survey metagenomic data set compared with 39 sequenced isolates indicated that natural Roseobacter populations differ systematically in several genomic attributes from their cultured representatives , including fewer genes for signal transduction and cell surface modifications but more genes for Sec-like protein secretion systems , anaplerotic CO ( 2 ) incorporation , and phosphorus and sulfate uptake .
	manualset3
246908	12	426359	16	NULL	NULL	0	NULL	genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in gene stoichiometry in the Global Ocean Survey metagenomic data set compared with 39 sequenced isolates indicated that natural Roseobacter populations differ systematically in several genomic attributes from their cultured representatives , including fewer genes for signal transduction and cell surface modifications but more genes for Sec-like protein secretion systems , anaplerotic CO ( 2 ) incorporation , and phosphorus and sulfate uptake .
	manualset3
246909	13	426359	16	NULL	NULL	NULL	NULL	Sec-like protein secretion systems	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differences in gene stoichiometry in the Global Ocean Survey metagenomic data set compared with 39 sequenced isolates indicated that natural Roseobacter populations differ systematically in several genomic attributes from their cultured representatives , including fewer genes for signal transduction and cell surface modifications but more genes for Sec-like protein secretion systems , anaplerotic CO ( 2 ) incorporation , and phosphorus and sulfate uptake .
	manualset3
246910	14	426359	16	NULL	NULL	NULL	NULL	anaplerotic CO ( 2 ) incorporation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differences in gene stoichiometry in the Global Ocean Survey metagenomic data set compared with 39 sequenced isolates indicated that natural Roseobacter populations differ systematically in several genomic attributes from their cultured representatives , including fewer genes for signal transduction and cell surface modifications but more genes for Sec-like protein secretion systems , anaplerotic CO ( 2 ) incorporation , and phosphorus and sulfate uptake .
	manualset3
246911	15	426359	16	NULL	NULL	NULL	NULL	phosphorus uptake	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differences in gene stoichiometry in the Global Ocean Survey metagenomic data set compared with 39 sequenced isolates indicated that natural Roseobacter populations differ systematically in several genomic attributes from their cultured representatives , including fewer genes for signal transduction and cell surface modifications but more genes for Sec-like protein secretion systems , anaplerotic CO ( 2 ) incorporation , and phosphorus and sulfate uptake .
	manualset3
246912	16	426359	16	NULL	NULL	NULL	NULL	sulfate uptake	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differences in gene stoichiometry in the Global Ocean Survey metagenomic data set compared with 39 sequenced isolates indicated that natural Roseobacter populations differ systematically in several genomic attributes from their cultured representatives , including fewer genes for signal transduction and cell surface modifications but more genes for Sec-like protein secretion systems , anaplerotic CO ( 2 ) incorporation , and phosphorus and sulfate uptake .
	manualset3
246913	1	426360	16	NULL	NULL	0	NULL	Differences	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in objective color measures and purge were minimal over the duration of storage time , but hams formulated with greater percentages of PSE raw materials were lighter in appearance and had less redness .
	manualset3
246914	2	426360	16	NULL	NULL	0	NULL	objective color measures	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in objective color measures and purge were minimal over the duration of storage time , but hams formulated with greater percentages of PSE raw materials were lighter in appearance and had less redness .
	manualset3
246915	3	426360	16	NULL	NULL	0	NULL	purge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in objective color measures and purge were minimal over the duration of storage time , but hams formulated with greater percentages of PSE raw materials were lighter in appearance and had less redness .
	manualset3
246916	4	426360	16	NULL	NULL	0	NULL	duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in objective color measures and purge were minimal over the duration of storage time , but hams formulated with greater percentages of PSE raw materials were lighter in appearance and had less redness .
	manualset3
246917	5	426360	16	NULL	NULL	0	NULL	storage time	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in objective color measures and purge were minimal over the duration of storage time , but hams formulated with greater percentages of PSE raw materials were lighter in appearance and had less redness .
	manualset3
247065	6	426360	16	NULL	NULL	0	NULL	hams	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in objective color measures and purge were minimal over the duration of storage time , but hams formulated with greater percentages of PSE raw materials were lighter in appearance and had less redness .
	manualset3
247066	7	426360	16	NULL	NULL	0	NULL	percentages	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in objective color measures and purge were minimal over the duration of storage time , but hams formulated with greater percentages of PSE raw materials were lighter in appearance and had less redness .
	manualset3
247067	8	426360	16	NULL	NULL	0	NULL	PSE raw materials	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in objective color measures and purge were minimal over the duration of storage time , but hams formulated with greater percentages of PSE raw materials were lighter in appearance and had less redness .
	manualset3
247071	9	426360	16	NULL	NULL	0	NULL	appearance	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in objective color measures and purge were minimal over the duration of storage time , but hams formulated with greater percentages of PSE raw materials were lighter in appearance and had less redness .
	manualset3
247072	10	426360	16	NULL	NULL	0	NULL	redness	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in objective color measures and purge were minimal over the duration of storage time , but hams formulated with greater percentages of PSE raw materials were lighter in appearance and had less redness .
	manualset3
247074	1	426361	16	NULL	NULL	0	NULL	Differences	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in phenotype and cell replicative behavior of hepatic tumors induced by dichloroacetate ( DCA ) and trichloroacetate ( TCA ) .
	manualset3
247077	2	426361	16	NULL	NULL	NULL	NULL	phenotype	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differences in phenotype and cell replicative behavior of hepatic tumors induced by dichloroacetate ( DCA ) and trichloroacetate ( TCA ) .
	manualset3
247078	3	426361	16	NULL	NULL	NULL	NULL	cell replicative behavior	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differences in phenotype and cell replicative behavior of hepatic tumors induced by dichloroacetate ( DCA ) and trichloroacetate ( TCA ) .
	manualset3
247079	4	426361	16	NULL	NULL	0	NULL	hepatic tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in phenotype and cell replicative behavior of hepatic tumors induced by dichloroacetate ( DCA ) and trichloroacetate ( TCA ) .
	manualset3
247080	5	426361	16	NULL	NULL	0	NULL	dichloroacetate ( DCA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in phenotype and cell replicative behavior of hepatic tumors induced by dichloroacetate ( DCA ) and trichloroacetate ( TCA ) .
	manualset3
247081	6	426361	16	NULL	NULL	0	NULL	trichloroacetate ( TCA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in phenotype and cell replicative behavior of hepatic tumors induced by dichloroacetate ( DCA ) and trichloroacetate ( TCA ) .
	manualset3
247128	1	426362	16	NULL	NULL	0	NULL	Differences	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in phorbol-ester-induced down-regulation of protein kinase C between cell lines .
	manualset3
247131	2	426362	16	NULL	NULL	NULL	NULL	phorbol-ester-induced down-regulation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differences in phorbol-ester-induced down-regulation of protein kinase C between cell lines .
	manualset3
247132	3	426362	16	NULL	NULL	NULL	NULL	protein kinase C	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differences in phorbol-ester-induced down-regulation of protein kinase C between cell lines .
	manualset3
247181	4	426362	16	NULL	NULL	0	NULL	 cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in phorbol-ester-induced down-regulation of protein kinase C between cell lines .
	manualset3
247183	1	426363	16	NULL	NULL	0	NULL	Differences	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in population characteristics , ( e.g. , age , conditions , co-morbidity ) , embedded within any cross-national trial , must be addressed conceptually prior to initiating the trial , methodologically when planning implementation , and statistically after the collection of the data .
	manualset3
247185	2	426363	16	NULL	NULL	0	NULL	population characteristics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in population characteristics , ( e.g. , age , conditions , co-morbidity ) , embedded within any cross-national trial , must be addressed conceptually prior to initiating the trial , methodologically when planning implementation , and statistically after the collection of the data .
	manualset3
247187	3	426363	16	NULL	NULL	0	NULL	age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in population characteristics , ( e.g. , age , conditions , co-morbidity ) , embedded within any cross-national trial , must be addressed conceptually prior to initiating the trial , methodologically when planning implementation , and statistically after the collection of the data .
	manualset3
247189	4	426363	16	NULL	NULL	0	NULL	conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in population characteristics , ( e.g. , age , conditions , co-morbidity ) , embedded within any cross-national trial , must be addressed conceptually prior to initiating the trial , methodologically when planning implementation , and statistically after the collection of the data .
	manualset3
247190	5	426363	16	NULL	NULL	0	NULL	co-morbidity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in population characteristics , ( e.g. , age , conditions , co-morbidity ) , embedded within any cross-national trial , must be addressed conceptually prior to initiating the trial , methodologically when planning implementation , and statistically after the collection of the data .
	manualset3
247191	6	426363	16	NULL	NULL	0	NULL	cross-national trial	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in population characteristics , ( e.g. , age , conditions , co-morbidity ) , embedded within any cross-national trial , must be addressed conceptually prior to initiating the trial , methodologically when planning implementation , and statistically after the collection of the data .
	manualset3
247247	7	426363	16	NULL	NULL	0	NULL	planning implementation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in population characteristics , ( e.g. , age , conditions , co-morbidity ) , embedded within any cross-national trial , must be addressed conceptually prior to initiating the trial , methodologically when planning implementation , and statistically after the collection of the data .
	manualset3
247248	8	426363	16	NULL	NULL	0	NULL	collection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in population characteristics , ( e.g. , age , conditions , co-morbidity ) , embedded within any cross-national trial , must be addressed conceptually prior to initiating the trial , methodologically when planning implementation , and statistically after the collection of the data .
	manualset3
247249	9	426363	16	NULL	NULL	0	NULL	data	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in population characteristics , ( e.g. , age , conditions , co-morbidity ) , embedded within any cross-national trial , must be addressed conceptually prior to initiating the trial , methodologically when planning implementation , and statistically after the collection of the data .
	manualset3
254093	10	426363	16	NULL	NULL	NULL	NULL	trial	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differences in population characteristics , ( e.g. , age , conditions , co-morbidity ) , embedded within any cross-national trial , must be addressed conceptually prior to initiating the trial , methodologically when planning implementation , and statistically after the collection of the data .
	manualset3
247250	1	426364	16	NULL	NULL	NULL	NULL	QUANTITATIVE DETERMINATION	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( ON THE QUANTITATIVE DETERMINATION OF PROTEASE INHIBITORS ) .
	manualset3
247251	2	426364	16	NULL	NULL	0	NULL	PROTEASE INHIBITORS	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( ON THE QUANTITATIVE DETERMINATION OF PROTEASE INHIBITORS ) .
	manualset3
247252	1	426365	16	NULL	NULL	0	NULL	Differences	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in signal transduction pathways by which platelet-derived and fibroblast growth factors activate extracellular signal-regulated kinase in differentiating oligodendrocytes .
	manualset3
247253	2	426365	16	NULL	NULL	NULL	NULL	signal transduction pathways	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differences in signal transduction pathways by which platelet-derived and fibroblast growth factors activate extracellular signal-regulated kinase in differentiating oligodendrocytes .
	manualset3
247254	3	426365	16	NULL	NULL	0	NULL	platelet-derived growth factors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in signal transduction pathways by which platelet-derived and fibroblast growth factors activate extracellular signal-regulated kinase in differentiating oligodendrocytes .
	manualset3
247255	4	426365	16	NULL	NULL	0	NULL	fibroblast growth factors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in signal transduction pathways by which platelet-derived and fibroblast growth factors activate extracellular signal-regulated kinase in differentiating oligodendrocytes .
	manualset3
247256	5	426365	16	NULL	NULL	0	NULL	 extracellular signal-regulated kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in signal transduction pathways by which platelet-derived and fibroblast growth factors activate extracellular signal-regulated kinase in differentiating oligodendrocytes .
	manualset3
247257	6	426365	16	NULL	NULL	0	NULL	differentiating oligodendrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in signal transduction pathways by which platelet-derived and fibroblast growth factors activate extracellular signal-regulated kinase in differentiating oligodendrocytes .
	manualset3
247258	1	426366	16	NULL	NULL	0	NULL	Differences	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in susceptibility to oxidative stress in the skin of Japanese and French subjects and physiological characteristics of their skin .
	manualset3
247259	2	426366	16	NULL	NULL	0	NULL	susceptibility to oxidative stress	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in susceptibility to oxidative stress in the skin of Japanese and French subjects and physiological characteristics of their skin .
	manualset3
247260	3	426366	16	NULL	NULL	0	NULL	skin	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in susceptibility to oxidative stress in the skin of Japanese and French subjects and physiological characteristics of their skin .
	manualset3
247261	4	426366	16	NULL	NULL	0	NULL	Japanese subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in susceptibility to oxidative stress in the skin of Japanese and French subjects and physiological characteristics of their skin .
	manualset3
247262	5	426366	16	NULL	NULL	0	NULL	French subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in susceptibility to oxidative stress in the skin of Japanese and French subjects and physiological characteristics of their skin .
	manualset3
247263	6	426366	16	NULL	NULL	0	NULL	physiological characteristics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in susceptibility to oxidative stress in the skin of Japanese and French subjects and physiological characteristics of their skin .
	manualset3
247264	7	426366	16	NULL	NULL	0	NULL	skin	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in susceptibility to oxidative stress in the skin of Japanese and French subjects and physiological characteristics of their skin .
	manualset3
247265	1	426367	16	NULL	NULL	0	NULL	Differences	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in the seasonal variation in stem water potential between the two shrub species Sorbus aucuparia and Sambucus nigra were related with their vulnerability to xylem cavitation .
	manualset3
247266	2	426367	16	NULL	NULL	NULL	NULL	seasonal variation	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differences in the seasonal variation in stem water potential between the two shrub species Sorbus aucuparia and Sambucus nigra were related with their vulnerability to xylem cavitation .
	manualset3
247267	3	426367	16	NULL	NULL	0	NULL	stem water potential	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in the seasonal variation in stem water potential between the two shrub species Sorbus aucuparia and Sambucus nigra were related with their vulnerability to xylem cavitation .
	manualset3
247268	4	426367	16	NULL	NULL	NULL	NULL	two shrub species	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differences in the seasonal variation in stem water potential between the two shrub species Sorbus aucuparia and Sambucus nigra were related with their vulnerability to xylem cavitation .
	manualset3
247269	5	426367	16	NULL	NULL	0	NULL	Sorbus aucuparia	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in the seasonal variation in stem water potential between the two shrub species Sorbus aucuparia and Sambucus nigra were related with their vulnerability to xylem cavitation .
	manualset3
247270	6	426367	16	NULL	NULL	0	NULL	Sambucus nigra	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in the seasonal variation in stem water potential between the two shrub species Sorbus aucuparia and Sambucus nigra were related with their vulnerability to xylem cavitation .
	manualset3
247271	7	426367	16	NULL	NULL	0	NULL	vulnerability to xylem cavitation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences in the seasonal variation in stem water potential between the two shrub species Sorbus aucuparia and Sambucus nigra were related with their vulnerability to xylem cavitation .
	manualset3
247272	1	426368	16	NULL	NULL	0	NULL	Differences	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences were examined in Theory of Planned Behaviour determinants of students ' intention to smoke including parents ' attitudes towards smoking and parents ' current cigarette use among Greek students of different school grade levels .
	manualset3
247273	2	426368	16	NULL	NULL	0	NULL	Theory of Planned Behaviour determinants	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences were examined in Theory of Planned Behaviour determinants of students ' intention to smoke including parents ' attitudes towards smoking and parents ' current cigarette use among Greek students of different school grade levels .
	manualset3
247274	3	426368	16	NULL	NULL	0	NULL	students	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences were examined in Theory of Planned Behaviour determinants of students ' intention to smoke including parents ' attitudes towards smoking and parents ' current cigarette use among Greek students of different school grade levels .
	manualset3
247275	4	426368	16	NULL	NULL	0	NULL	intention to smoke	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences were examined in Theory of Planned Behaviour determinants of students ' intention to smoke including parents ' attitudes towards smoking and parents ' current cigarette use among Greek students of different school grade levels .
	manualset3
247615	5	426368	16	NULL	NULL	0	NULL	parents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences were examined in Theory of Planned Behaviour determinants of students ' intention to smoke including parents ' attitudes towards smoking and parents ' current cigarette use among Greek students of different school grade levels .
	manualset3
247616	6	426368	16	NULL	NULL	0	NULL	attitudes	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences were examined in Theory of Planned Behaviour determinants of students ' intention to smoke including parents ' attitudes towards smoking and parents ' current cigarette use among Greek students of different school grade levels .
	manualset3
247617	7	426368	16	NULL	NULL	0	NULL	smoking	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences were examined in Theory of Planned Behaviour determinants of students ' intention to smoke including parents ' attitudes towards smoking and parents ' current cigarette use among Greek students of different school grade levels .
	manualset3
247618	8	426368	16	NULL	NULL	0	NULL	parents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences were examined in Theory of Planned Behaviour determinants of students ' intention to smoke including parents ' attitudes towards smoking and parents ' current cigarette use among Greek students of different school grade levels .
	manualset3
247619	9	426368	16	NULL	NULL	0	NULL	current cigarette use	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences were examined in Theory of Planned Behaviour determinants of students ' intention to smoke including parents ' attitudes towards smoking and parents ' current cigarette use among Greek students of different school grade levels .
	manualset3
247620	10	426368	16	NULL	NULL	0	NULL	Greek students	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences were examined in Theory of Planned Behaviour determinants of students ' intention to smoke including parents ' attitudes towards smoking and parents ' current cigarette use among Greek students of different school grade levels .
	manualset3
247621	11	426368	16	NULL	NULL	0	NULL	school	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences were examined in Theory of Planned Behaviour determinants of students ' intention to smoke including parents ' attitudes towards smoking and parents ' current cigarette use among Greek students of different school grade levels .
	manualset3
247622	12	426368	16	NULL	NULL	0	NULL	grade levels	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences were examined in Theory of Planned Behaviour determinants of students ' intention to smoke including parents ' attitudes towards smoking and parents ' current cigarette use among Greek students of different school grade levels .
	manualset3
247276	1	426369	16	NULL	NULL	0	NULL	Differences	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences were partially restored in the presence of growth factors or serum .
	manualset3
247277	2	426369	16	NULL	NULL	0	NULL	presence	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences were partially restored in the presence of growth factors or serum .
	manualset3
247278	3	426369	16	NULL	NULL	0	NULL	growth factors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Differences were partially restored in the presence of growth factors or serum .
	manualset3
247279	4	426369	16	NULL	NULL	NULL	NULL	serum	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differences were partially restored in the presence of growth factors or serum .
	manualset3
247280	1	426370	16	NULL	NULL	0	NULL	4 ' - alkyl substituents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Different 4 ' - alkyl , 4 ' - alkenyl , and 4 ' - alkynyl substituents were introduced in the phenyl ring of the benzyl moiety along with the replacement of the same phenyl ring by the isomeric alpha - and beta-naphthyl groups .
	manualset3
247281	2	426370	16	NULL	NULL	0	NULL	4 ' - alkenyl substituents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Different 4 ' - alkyl , 4 ' - alkenyl , and 4 ' - alkynyl substituents were introduced in the phenyl ring of the benzyl moiety along with the replacement of the same phenyl ring by the isomeric alpha - and beta-naphthyl groups .
	manualset3
247282	3	426370	16	NULL	NULL	0	NULL	4 ' - alkynyl substituents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Different 4 ' - alkyl , 4 ' - alkenyl , and 4 ' - alkynyl substituents were introduced in the phenyl ring of the benzyl moiety along with the replacement of the same phenyl ring by the isomeric alpha - and beta-naphthyl groups .
	manualset3
247283	4	426370	16	NULL	NULL	0	NULL	phenyl ring	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Different 4 ' - alkyl , 4 ' - alkenyl , and 4 ' - alkynyl substituents were introduced in the phenyl ring of the benzyl moiety along with the replacement of the same phenyl ring by the isomeric alpha - and beta-naphthyl groups .
	manualset3
247284	5	426370	16	NULL	NULL	0	NULL	benzyl moiety	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Different 4 ' - alkyl , 4 ' - alkenyl , and 4 ' - alkynyl substituents were introduced in the phenyl ring of the benzyl moiety along with the replacement of the same phenyl ring by the isomeric alpha - and beta-naphthyl groups .
	manualset3
247285	6	426370	16	NULL	NULL	0	NULL	replacement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Different 4 ' - alkyl , 4 ' - alkenyl , and 4 ' - alkynyl substituents were introduced in the phenyl ring of the benzyl moiety along with the replacement of the same phenyl ring by the isomeric alpha - and beta-naphthyl groups .
	manualset3
247286	7	426370	16	NULL	NULL	0	NULL	phenyl ring	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Different 4 ' - alkyl , 4 ' - alkenyl , and 4 ' - alkynyl substituents were introduced in the phenyl ring of the benzyl moiety along with the replacement of the same phenyl ring by the isomeric alpha - and beta-naphthyl groups .
	manualset3
247287	8	426370	16	NULL	NULL	0	NULL	isomeric alpha groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Different 4 ' - alkyl , 4 ' - alkenyl , and 4 ' - alkynyl substituents were introduced in the phenyl ring of the benzyl moiety along with the replacement of the same phenyl ring by the isomeric alpha - and beta-naphthyl groups .
	manualset3
247288	9	426370	16	NULL	NULL	0	NULL	beta-naphthyl groups	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Different 4 ' - alkyl , 4 ' - alkenyl , and 4 ' - alkynyl substituents were introduced in the phenyl ring of the benzyl moiety along with the replacement of the same phenyl ring by the isomeric alpha - and beta-naphthyl groups .
	manualset3
247289	1	426371	16	NULL	NULL	0	NULL	HpaI digestion patterns	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Different HpaI digestion patterns were observed for plasmids , but all of them belonged to IncFIB group and harboured bla ( CTX-M-15 ) associated with bla ( OXA-1 ) , bla ( TEM ) , tetA , catB3 and aac ( 6 ' ) - Ib surrounded by an identical genetic environment .
	manualset3
247290	2	426371	16	NULL	NULL	0	NULL	plasmids	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Different HpaI digestion patterns were observed for plasmids , but all of them belonged to IncFIB group and harboured bla ( CTX-M-15 ) associated with bla ( OXA-1 ) , bla ( TEM ) , tetA , catB3 and aac ( 6 ' ) - Ib surrounded by an identical genetic environment .
	manualset3
247291	3	426371	16	NULL	NULL	NULL	NULL	IncFIB group	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Different HpaI digestion patterns were observed for plasmids , but all of them belonged to IncFIB group and harboured bla ( CTX-M-15 ) associated with bla ( OXA-1 ) , bla ( TEM ) , tetA , catB3 and aac ( 6 ' ) - Ib surrounded by an identical genetic environment .
	manualset3
247292	4	426371	16	NULL	NULL	0	NULL	bla ( CTX-M-15 )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Different HpaI digestion patterns were observed for plasmids , but all of them belonged to IncFIB group and harboured bla ( CTX-M-15 ) associated with bla ( OXA-1 ) , bla ( TEM ) , tetA , catB3 and aac ( 6 ' ) - Ib surrounded by an identical genetic environment .
	manualset3
247293	5	426371	16	NULL	NULL	0	NULL	bla ( OXA-1 )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Different HpaI digestion patterns were observed for plasmids , but all of them belonged to IncFIB group and harboured bla ( CTX-M-15 ) associated with bla ( OXA-1 ) , bla ( TEM ) , tetA , catB3 and aac ( 6 ' ) - Ib surrounded by an identical genetic environment .
	manualset3
247294	6	426371	16	NULL	NULL	0	NULL	 bla ( TEM )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Different HpaI digestion patterns were observed for plasmids , but all of them belonged to IncFIB group and harboured bla ( CTX-M-15 ) associated with bla ( OXA-1 ) , bla ( TEM ) , tetA , catB3 and aac ( 6 ' ) - Ib surrounded by an identical genetic environment .
	manualset3
247295	7	426371	16	NULL	NULL	0	NULL	tetA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Different HpaI digestion patterns were observed for plasmids , but all of them belonged to IncFIB group and harboured bla ( CTX-M-15 ) associated with bla ( OXA-1 ) , bla ( TEM ) , tetA , catB3 and aac ( 6 ' ) - Ib surrounded by an identical genetic environment .
	manualset3
247296	8	426371	16	NULL	NULL	0	NULL	catB3	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Different HpaI digestion patterns were observed for plasmids , but all of them belonged to IncFIB group and harboured bla ( CTX-M-15 ) associated with bla ( OXA-1 ) , bla ( TEM ) , tetA , catB3 and aac ( 6 ' ) - Ib surrounded by an identical genetic environment .
	manualset3
247297	9	426371	16	NULL	NULL	0	NULL	aac ( 6 ' ) - Ib	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Different HpaI digestion patterns were observed for plasmids , but all of them belonged to IncFIB group and harboured bla ( CTX-M-15 ) associated with bla ( OXA-1 ) , bla ( TEM ) , tetA , catB3 and aac ( 6 ' ) - Ib surrounded by an identical genetic environment .
	manualset3
247298	10	426371	16	NULL	NULL	0	NULL	genetic environment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Different HpaI digestion patterns were observed for plasmids , but all of them belonged to IncFIB group and harboured bla ( CTX-M-15 ) associated with bla ( OXA-1 ) , bla ( TEM ) , tetA , catB3 and aac ( 6 ' ) - Ib surrounded by an identical genetic environment .
	manualset3
247299	1	426372	16	NULL	NULL	0	NULL	chemical treatments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Different chemical treatments were applied to solutions of Aflatoxin B1 in order to compare their efficacy for the detoxification of AfB1 : sodium sulfite , sodium hydrogen sulfate , sodium hydroxide , ammonia , sodium hypochlorite , hydrogen peroxide .
	manualset3
247300	2	426372	16	NULL	NULL	0	NULL	solutions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Different chemical treatments were applied to solutions of Aflatoxin B1 in order to compare their efficacy for the detoxification of AfB1 : sodium sulfite , sodium hydrogen sulfate , sodium hydroxide , ammonia , sodium hypochlorite , hydrogen peroxide .
	manualset3
247301	3	426372	16	NULL	NULL	0	NULL	Aflatoxin B1	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Different chemical treatments were applied to solutions of Aflatoxin B1 in order to compare their efficacy for the detoxification of AfB1 : sodium sulfite , sodium hydrogen sulfate , sodium hydroxide , ammonia , sodium hypochlorite , hydrogen peroxide .
	manualset3
247302	4	426372	16	NULL	NULL	NULL	NULL	efficacy	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Different chemical treatments were applied to solutions of Aflatoxin B1 in order to compare their efficacy for the detoxification of AfB1 : sodium sulfite , sodium hydrogen sulfate , sodium hydroxide , ammonia , sodium hypochlorite , hydrogen peroxide .
	manualset3
247303	5	426372	16	NULL	NULL	NULL	NULL	detoxification	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Different chemical treatments were applied to solutions of Aflatoxin B1 in order to compare their efficacy for the detoxification of AfB1 : sodium sulfite , sodium hydrogen sulfate , sodium hydroxide , ammonia , sodium hypochlorite , hydrogen peroxide .
	manualset3
247304	6	426372	16	NULL	NULL	0	NULL	AfB1	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Different chemical treatments were applied to solutions of Aflatoxin B1 in order to compare their efficacy for the detoxification of AfB1 : sodium sulfite , sodium hydrogen sulfate , sodium hydroxide , ammonia , sodium hypochlorite , hydrogen peroxide .
	manualset3
247305	7	426372	16	NULL	NULL	0	NULL	sodium sulfite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Different chemical treatments were applied to solutions of Aflatoxin B1 in order to compare their efficacy for the detoxification of AfB1 : sodium sulfite , sodium hydrogen sulfate , sodium hydroxide , ammonia , sodium hypochlorite , hydrogen peroxide .
	manualset3
247306	8	426372	16	NULL	NULL	0	NULL	sodium hydrogen sulfate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Different chemical treatments were applied to solutions of Aflatoxin B1 in order to compare their efficacy for the detoxification of AfB1 : sodium sulfite , sodium hydrogen sulfate , sodium hydroxide , ammonia , sodium hypochlorite , hydrogen peroxide .
	manualset3
247307	9	426372	16	NULL	NULL	0	NULL	sodium hydroxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Different chemical treatments were applied to solutions of Aflatoxin B1 in order to compare their efficacy for the detoxification of AfB1 : sodium sulfite , sodium hydrogen sulfate , sodium hydroxide , ammonia , sodium hypochlorite , hydrogen peroxide .
	manualset3
247308	10	426372	16	NULL	NULL	0	NULL	ammonia	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Different chemical treatments were applied to solutions of Aflatoxin B1 in order to compare their efficacy for the detoxification of AfB1 : sodium sulfite , sodium hydrogen sulfate , sodium hydroxide , ammonia , sodium hypochlorite , hydrogen peroxide .
	manualset3
247309	11	426372	16	NULL	NULL	0	NULL	sodium hypochlorite	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Different chemical treatments were applied to solutions of Aflatoxin B1 in order to compare their efficacy for the detoxification of AfB1 : sodium sulfite , sodium hydrogen sulfate , sodium hydroxide , ammonia , sodium hypochlorite , hydrogen peroxide .
	manualset3
247310	12	426372	16	NULL	NULL	0	NULL	hydrogen peroxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Different chemical treatments were applied to solutions of Aflatoxin B1 in order to compare their efficacy for the detoxification of AfB1 : sodium sulfite , sodium hydrogen sulfate , sodium hydroxide , ammonia , sodium hypochlorite , hydrogen peroxide .
	manualset3
247311	1	426373	16	NULL	NULL	0	NULL	PHYSIOLOGICAL CHANGES	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( ON SOME PHYSIOLOGICAL CHANGES IN THE ELECTROCARDIOGRAM OF THE RAT : RESPIRATORY CHANGES AND THOSE DUE TO CHANGES OF POSTURE ) .
	manualset3
247312	2	426373	16	NULL	NULL	0	NULL	ELECTROCARDIOGRAM	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( ON SOME PHYSIOLOGICAL CHANGES IN THE ELECTROCARDIOGRAM OF THE RAT : RESPIRATORY CHANGES AND THOSE DUE TO CHANGES OF POSTURE ) .
	manualset3
247313	3	426373	16	NULL	NULL	0	NULL	RAT	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( ON SOME PHYSIOLOGICAL CHANGES IN THE ELECTROCARDIOGRAM OF THE RAT : RESPIRATORY CHANGES AND THOSE DUE TO CHANGES OF POSTURE ) .
	manualset3
247314	4	426373	16	NULL	NULL	0	NULL	RESPIRATORY CHANGES	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( ON SOME PHYSIOLOGICAL CHANGES IN THE ELECTROCARDIOGRAM OF THE RAT : RESPIRATORY CHANGES AND THOSE DUE TO CHANGES OF POSTURE ) .
	manualset3
247315	5	426373	16	NULL	NULL	0	NULL	CHANGES OF POSTURE	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( ON SOME PHYSIOLOGICAL CHANGES IN THE ELECTROCARDIOGRAM OF THE RAT : RESPIRATORY CHANGES AND THOSE DUE TO CHANGES OF POSTURE ) .
	manualset3
247316	1	426374	16	NULL	NULL	0	NULL	correlates	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Different correlates of GAF score were found between suicides and controls .
	manualset3
247317	2	426374	16	NULL	NULL	0	NULL	GAF score	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Different correlates of GAF score were found between suicides and controls .
	manualset3
247318	3	426374	16	NULL	NULL	0	NULL	suicides	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Different correlates of GAF score were found between suicides and controls .
	manualset3
247319	4	426374	16	NULL	NULL	0	NULL	controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Different correlates of GAF score were found between suicides and controls .
	manualset3
247320	1	426375	16	NULL	NULL	NULL	NULL	earlier suggestions	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Different from some earlier suggestions , zinc has no difficulty in accepting an activated substrate as the fifth ligand to switch from tetra - to penta-coordination in either PDF or TLN .
	manualset3
247321	2	426375	16	NULL	NULL	0	NULL	zinc	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Different from some earlier suggestions , zinc has no difficulty in accepting an activated substrate as the fifth ligand to switch from tetra - to penta-coordination in either PDF or TLN .
	manualset3
247322	3	426375	16	NULL	NULL	NULL	NULL	difficulty	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Different from some earlier suggestions , zinc has no difficulty in accepting an activated substrate as the fifth ligand to switch from tetra - to penta-coordination in either PDF or TLN .
	manualset3
247323	4	426375	16	NULL	NULL	0	NULL	activated substrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Different from some earlier suggestions , zinc has no difficulty in accepting an activated substrate as the fifth ligand to switch from tetra - to penta-coordination in either PDF or TLN .
	manualset3
247324	5	426375	16	NULL	NULL	0	NULL	fifth ligand	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Different from some earlier suggestions , zinc has no difficulty in accepting an activated substrate as the fifth ligand to switch from tetra - to penta-coordination in either PDF or TLN .
	manualset3
247325	6	426375	16	NULL	NULL	0	NULL	tetra-coordination	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Different from some earlier suggestions , zinc has no difficulty in accepting an activated substrate as the fifth ligand to switch from tetra - to penta-coordination in either PDF or TLN .
	manualset3
247326	7	426375	16	NULL	NULL	0	NULL	penta-coordination	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Different from some earlier suggestions , zinc has no difficulty in accepting an activated substrate as the fifth ligand to switch from tetra - to penta-coordination in either PDF or TLN .
	manualset3
247327	8	426375	16	NULL	NULL	0	NULL	PDF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Different from some earlier suggestions , zinc has no difficulty in accepting an activated substrate as the fifth ligand to switch from tetra - to penta-coordination in either PDF or TLN .
	manualset3
247328	9	426375	16	NULL	NULL	0	NULL	TLN	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Different from some earlier suggestions , zinc has no difficulty in accepting an activated substrate as the fifth ligand to switch from tetra - to penta-coordination in either PDF or TLN .
	manualset3
247332	1	426377	16	NULL	NULL	0	NULL	estimates	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Different possible estimates of the intake are considered : some represent the parameters of the PDF of the output quantity , others are derived from the commonly used constant chronic , I ( CC ) , and mid-point , I ( 1/2 ) , methods .
	manualset3
247333	2	426377	16	NULL	NULL	0	NULL	intake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Different possible estimates of the intake are considered : some represent the parameters of the PDF of the output quantity , others are derived from the commonly used constant chronic , I ( CC ) , and mid-point , I ( 1/2 ) , methods .
	manualset3
247334	3	426377	16	NULL	NULL	NULL	NULL	parameters	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Different possible estimates of the intake are considered : some represent the parameters of the PDF of the output quantity , others are derived from the commonly used constant chronic , I ( CC ) , and mid-point , I ( 1/2 ) , methods .
	manualset3
247335	4	426377	16	NULL	NULL	0	NULL	PDF	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Different possible estimates of the intake are considered : some represent the parameters of the PDF of the output quantity , others are derived from the commonly used constant chronic , I ( CC ) , and mid-point , I ( 1/2 ) , methods .
	manualset3
247336	5	426377	16	NULL	NULL	0	NULL	output quantity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Different possible estimates of the intake are considered : some represent the parameters of the PDF of the output quantity , others are derived from the commonly used constant chronic , I ( CC ) , and mid-point , I ( 1/2 ) , methods .
	manualset3
247337	6	426377	16	NULL	NULL	0	NULL	others	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Different possible estimates of the intake are considered : some represent the parameters of the PDF of the output quantity , others are derived from the commonly used constant chronic , I ( CC ) , and mid-point , I ( 1/2 ) , methods .
	manualset3
247338	7	426377	16	NULL	NULL	0	NULL	constant chronic methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Different possible estimates of the intake are considered : some represent the parameters of the PDF of the output quantity , others are derived from the commonly used constant chronic , I ( CC ) , and mid-point , I ( 1/2 ) , methods .
	manualset3
247339	8	426377	16	NULL	NULL	0	NULL	I ( CC ) methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Different possible estimates of the intake are considered : some represent the parameters of the PDF of the output quantity , others are derived from the commonly used constant chronic , I ( CC ) , and mid-point , I ( 1/2 ) , methods .
	manualset3
247340	9	426377	16	NULL	NULL	NULL	NULL	mid-point methods	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Different possible estimates of the intake are considered : some represent the parameters of the PDF of the output quantity , others are derived from the commonly used constant chronic , I ( CC ) , and mid-point , I ( 1/2 ) , methods .
	manualset3
247342	10	426377	16	NULL	NULL	0	NULL	I ( 1/2 ) , methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Different possible estimates of the intake are considered : some represent the parameters of the PDF of the output quantity , others are derived from the commonly used constant chronic , I ( CC ) , and mid-point , I ( 1/2 ) , methods .
	manualset3
247341	1	426378	16	NULL	NULL	NULL	NULL	psychological protective factors	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Different psychological , social and ecological protective factors , particularly competence , optimism , and bonding to family and cultural beliefs are highlighted .
	manualset3
247344	2	426378	16	NULL	NULL	0	NULL	social protective factors	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Different psychological , social and ecological protective factors , particularly competence , optimism , and bonding to family and cultural beliefs are highlighted .
	manualset3
247345	3	426378	16	NULL	NULL	0	NULL	ecological protective factors	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Different psychological , social and ecological protective factors , particularly competence , optimism , and bonding to family and cultural beliefs are highlighted .
	manualset3
247346	4	426378	16	NULL	NULL	0	NULL	competence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Different psychological , social and ecological protective factors , particularly competence , optimism , and bonding to family and cultural beliefs are highlighted .
	manualset3
247347	5	426378	16	NULL	NULL	0	NULL	optimism	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Different psychological , social and ecological protective factors , particularly competence , optimism , and bonding to family and cultural beliefs are highlighted .
	manualset3
247348	6	426378	16	NULL	NULL	0	NULL	bonding to family	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Different psychological , social and ecological protective factors , particularly competence , optimism , and bonding to family and cultural beliefs are highlighted .
	manualset3
247349	7	426378	16	NULL	NULL	0	NULL	cultural beliefs	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Different psychological , social and ecological protective factors , particularly competence , optimism , and bonding to family and cultural beliefs are highlighted .
	manualset3
247350	1	426379	16	NULL	NULL	0	NULL	rates	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Different rates of cellular uptake also may play a role in time course of toxicity of the cysteine conjugates and the mercapturic acids in the renal cells .
	manualset3
247351	2	426379	16	NULL	NULL	0	NULL	cellular uptake	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Different rates of cellular uptake also may play a role in time course of toxicity of the cysteine conjugates and the mercapturic acids in the renal cells .
	manualset3
247352	3	426379	16	NULL	NULL	NULL	NULL	role	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Different rates of cellular uptake also may play a role in time course of toxicity of the cysteine conjugates and the mercapturic acids in the renal cells .
	manualset3
247354	5	426379	16	NULL	NULL	NULL	NULL	time course	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Different rates of cellular uptake also may play a role in time course of toxicity of the cysteine conjugates and the mercapturic acids in the renal cells .
	manualset3
247355	6	426379	16	NULL	NULL	0	NULL	cysteine conjugates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Different rates of cellular uptake also may play a role in time course of toxicity of the cysteine conjugates and the mercapturic acids in the renal cells .
	manualset3
247356	7	426379	16	NULL	NULL	0	NULL	mercapturic acids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Different rates of cellular uptake also may play a role in time course of toxicity of the cysteine conjugates and the mercapturic acids in the renal cells .
	manualset3
247357	8	426379	16	NULL	NULL	0	NULL	renal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Different rates of cellular uptake also may play a role in time course of toxicity of the cysteine conjugates and the mercapturic acids in the renal cells .
	manualset3
255706	9	426379	16	NULL	NULL	NULL	NULL	toxicity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Different rates of cellular uptake also may play a role in time course of toxicity of the cysteine conjugates and the mercapturic acids in the renal cells .
	manualset3
247358	1	426380	16	NULL	NULL	0	NULL	spacer lengths	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Different spacer lengths and chelating systems have been introduced at these sites .
	manualset3
247359	2	426380	16	NULL	NULL	0	NULL	chelating systems	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Different spacer lengths and chelating systems have been introduced at these sites .
	manualset3
247360	3	426380	16	NULL	NULL	0	NULL	sites	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Different spacer lengths and chelating systems have been introduced at these sites .
	manualset3
247361	1	426381	16	NULL	NULL	0	NULL	temporal expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Different temporal expression of three wheat cystatin genes , WC2 , WC3 and WCMD was observed with their increased expression at 1DAI in the boot emergence stage which is most susceptible to KB and then slowly declined gradually at 3 , 7 and 15 DAI in both the varieties .
	manualset3
247362	2	426381	16	NULL	NULL	NULL	NULL	three wheat cystatin genes	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Different temporal expression of three wheat cystatin genes , WC2 , WC3 and WCMD was observed with their increased expression at 1DAI in the boot emergence stage which is most susceptible to KB and then slowly declined gradually at 3 , 7 and 15 DAI in both the varieties .
	manualset3
247363	3	426381	16	NULL	NULL	0	NULL	 WC2	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Different temporal expression of three wheat cystatin genes , WC2 , WC3 and WCMD was observed with their increased expression at 1DAI in the boot emergence stage which is most susceptible to KB and then slowly declined gradually at 3 , 7 and 15 DAI in both the varieties .
	manualset3
247364	4	426381	16	NULL	NULL	0	NULL	WC3	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Different temporal expression of three wheat cystatin genes , WC2 , WC3 and WCMD was observed with their increased expression at 1DAI in the boot emergence stage which is most susceptible to KB and then slowly declined gradually at 3 , 7 and 15 DAI in both the varieties .
	manualset3
247365	5	426381	16	NULL	NULL	0	NULL	WCMD	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Different temporal expression of three wheat cystatin genes , WC2 , WC3 and WCMD was observed with their increased expression at 1DAI in the boot emergence stage which is most susceptible to KB and then slowly declined gradually at 3 , 7 and 15 DAI in both the varieties .
	manualset3
247366	6	426381	16	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Different temporal expression of three wheat cystatin genes , WC2 , WC3 and WCMD was observed with their increased expression at 1DAI in the boot emergence stage which is most susceptible to KB and then slowly declined gradually at 3 , 7 and 15 DAI in both the varieties .
	manualset3
247367	7	426381	16	NULL	NULL	NULL	NULL	1DAI 	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Different temporal expression of three wheat cystatin genes , WC2 , WC3 and WCMD was observed with their increased expression at 1DAI in the boot emergence stage which is most susceptible to KB and then slowly declined gradually at 3 , 7 and 15 DAI in both the varieties .
	manualset3
247368	8	426381	16	NULL	NULL	NULL	NULL	boot emergence stage	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Different temporal expression of three wheat cystatin genes , WC2 , WC3 and WCMD was observed with their increased expression at 1DAI in the boot emergence stage which is most susceptible to KB and then slowly declined gradually at 3 , 7 and 15 DAI in both the varieties .
	manualset3
247369	9	426381	16	NULL	NULL	NULL	NULL	KB	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Different temporal expression of three wheat cystatin genes , WC2 , WC3 and WCMD was observed with their increased expression at 1DAI in the boot emergence stage which is most susceptible to KB and then slowly declined gradually at 3 , 7 and 15 DAI in both the varieties .
	manualset3
247370	10	426381	16	NULL	NULL	0	NULL	3 DAI	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Different temporal expression of three wheat cystatin genes , WC2 , WC3 and WCMD was observed with their increased expression at 1DAI in the boot emergence stage which is most susceptible to KB and then slowly declined gradually at 3 , 7 and 15 DAI in both the varieties .
	manualset3
247371	11	426381	16	NULL	NULL	0	NULL	7 DAI	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Different temporal expression of three wheat cystatin genes , WC2 , WC3 and WCMD was observed with their increased expression at 1DAI in the boot emergence stage which is most susceptible to KB and then slowly declined gradually at 3 , 7 and 15 DAI in both the varieties .
	manualset3
247373	12	426381	16	NULL	NULL	0	NULL	15 DAI	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Different temporal expression of three wheat cystatin genes , WC2 , WC3 and WCMD was observed with their increased expression at 1DAI in the boot emergence stage which is most susceptible to KB and then slowly declined gradually at 3 , 7 and 15 DAI in both the varieties .
	manualset3
247374	13	426381	16	NULL	NULL	NULL	NULL	varieties	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Different temporal expression of three wheat cystatin genes , WC2 , WC3 and WCMD was observed with their increased expression at 1DAI in the boot emergence stage which is most susceptible to KB and then slowly declined gradually at 3 , 7 and 15 DAI in both the varieties .
	manualset3
247378	1	426382	16	NULL	NULL	0	NULL	types of memory	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Different types of memory ( reference and working memory ) and/or information processing ( route or place learning ) were assessed in three different tasks ( T-maze , Morris water maze , and eight-arm radial maze ) .
	manualset3
247379	2	426382	16	NULL	NULL	0	NULL	reference memory	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Different types of memory ( reference and working memory ) and/or information processing ( route or place learning ) were assessed in three different tasks ( T-maze , Morris water maze , and eight-arm radial maze ) .
	manualset3
247381	3	426382	16	NULL	NULL	0	NULL	working memory	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Different types of memory ( reference and working memory ) and/or information processing ( route or place learning ) were assessed in three different tasks ( T-maze , Morris water maze , and eight-arm radial maze ) .
	manualset3
247382	4	426382	16	NULL	NULL	0	NULL	information processing	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Different types of memory ( reference and working memory ) and/or information processing ( route or place learning ) were assessed in three different tasks ( T-maze , Morris water maze , and eight-arm radial maze ) .
	manualset3
247383	5	426382	16	NULL	NULL	0	NULL	route learning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Different types of memory ( reference and working memory ) and/or information processing ( route or place learning ) were assessed in three different tasks ( T-maze , Morris water maze , and eight-arm radial maze ) .
	manualset3
247384	6	426382	16	NULL	NULL	0	NULL	place learning	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Different types of memory ( reference and working memory ) and/or information processing ( route or place learning ) were assessed in three different tasks ( T-maze , Morris water maze , and eight-arm radial maze ) .
	manualset3
247385	7	426382	16	NULL	NULL	NULL	NULL	three	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Different types of memory ( reference and working memory ) and/or information processing ( route or place learning ) were assessed in three different tasks ( T-maze , Morris water maze , and eight-arm radial maze ) .
	manualset3
247386	8	426382	16	NULL	NULL	0	NULL	 T-maze 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Different types of memory ( reference and working memory ) and/or information processing ( route or place learning ) were assessed in three different tasks ( T-maze , Morris water maze , and eight-arm radial maze ) .
	manualset3
247387	9	426382	16	NULL	NULL	0	NULL	Morris water maze	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Different types of memory ( reference and working memory ) and/or information processing ( route or place learning ) were assessed in three different tasks ( T-maze , Morris water maze , and eight-arm radial maze ) .
	manualset3
247388	10	426382	16	NULL	NULL	0	NULL	eight-arm radial maze	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Different types of memory ( reference and working memory ) and/or information processing ( route or place learning ) were assessed in three different tasks ( T-maze , Morris water maze , and eight-arm radial maze ) .
	manualset3
255726	11	426382	16	NULL	NULL	NULL	NULL	tasks	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Different types of memory ( reference and working memory ) and/or information processing ( route or place learning ) were assessed in three different tasks ( T-maze , Morris water maze , and eight-arm radial maze ) .
	manualset3
247391	1	426383	16	NULL	NULL	0	NULL	Differential diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential diagnosis is concerned with various forms of intersexuality , especially aplasia and atresia of the vagina .
	manualset3
247393	2	426383	16	NULL	NULL	0	NULL	various forms	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential diagnosis is concerned with various forms of intersexuality , especially aplasia and atresia of the vagina .
	manualset3
247395	3	426383	16	NULL	NULL	0	NULL	intersexuality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential diagnosis is concerned with various forms of intersexuality , especially aplasia and atresia of the vagina .
	manualset3
247396	4	426383	16	NULL	NULL	NULL	NULL	aplasia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differential diagnosis is concerned with various forms of intersexuality , especially aplasia and atresia of the vagina .
	manualset3
247397	5	426383	16	NULL	NULL	NULL	NULL	atresia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differential diagnosis is concerned with various forms of intersexuality , especially aplasia and atresia of the vagina .
	manualset3
255733	6	426383	16	NULL	NULL	NULL	NULL	vagina	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differential diagnosis is concerned with various forms of intersexuality , especially aplasia and atresia of the vagina .
	manualset3
247407	1	426384	16	NULL	NULL	NULL	NULL	Differential effect	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differential effect of the 5-HTT gene-linked polymorphic region on emotional eating during stress exposure following tryptophan challenge .
	manualset3
247408	2	426384	16	NULL	NULL	0	NULL	5-HTT gene-linked polymorphic region	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential effect of the 5-HTT gene-linked polymorphic region on emotional eating during stress exposure following tryptophan challenge .
	manualset3
247409	3	426384	16	NULL	NULL	0	NULL	emotional eating	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential effect of the 5-HTT gene-linked polymorphic region on emotional eating during stress exposure following tryptophan challenge .
	manualset3
247410	4	426384	16	NULL	NULL	NULL	NULL	stress exposure	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differential effect of the 5-HTT gene-linked polymorphic region on emotional eating during stress exposure following tryptophan challenge .
	manualset3
247411	5	426384	16	NULL	NULL	0	NULL	tryptophan challenge	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential effect of the 5-HTT gene-linked polymorphic region on emotional eating during stress exposure following tryptophan challenge .
	manualset3
247412	1	426385	16	NULL	NULL	0	NULL	Differential effects	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential effects of TGF-1 and FGF-2 on SDF-1 expression in human periodontal ligament cells derived from deciduous teeth in vitro .
	manualset3
247413	2	426385	16	NULL	NULL	0	NULL	TGF-1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential effects of TGF-1 and FGF-2 on SDF-1 expression in human periodontal ligament cells derived from deciduous teeth in vitro .
	manualset3
247414	3	426385	16	NULL	NULL	0	NULL	FGF-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential effects of TGF-1 and FGF-2 on SDF-1 expression in human periodontal ligament cells derived from deciduous teeth in vitro .
	manualset3
247415	4	426385	16	NULL	NULL	0	NULL	SDF-1 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential effects of TGF-1 and FGF-2 on SDF-1 expression in human periodontal ligament cells derived from deciduous teeth in vitro .
	manualset3
247416	5	426385	16	NULL	NULL	0	NULL	human periodontal ligament cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential effects of TGF-1 and FGF-2 on SDF-1 expression in human periodontal ligament cells derived from deciduous teeth in vitro .
	manualset3
247417	6	426385	16	NULL	NULL	0	NULL	deciduous teeth	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential effects of TGF-1 and FGF-2 on SDF-1 expression in human periodontal ligament cells derived from deciduous teeth in vitro .
	manualset3
247419	1	426386	16	NULL	NULL	NULL	NULL	Differential electrophysiological features	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differential electrophysiological features of neuropathies associated with 17p11 .2 deletion and duplication .
	manualset3
247420	2	426386	16	NULL	NULL	0	NULL	neuropathies	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential electrophysiological features of neuropathies associated with 17p11 .2 deletion and duplication .
	manualset3
247421	3	426386	16	NULL	NULL	0	NULL	17p11 .2 deletion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential electrophysiological features of neuropathies associated with 17p11 .2 deletion and duplication .
	manualset3
247422	4	426386	16	NULL	NULL	0	NULL	17p11 .2  duplication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential electrophysiological features of neuropathies associated with 17p11 .2 deletion and duplication .
	manualset3
247426	1	426387	16	NULL	NULL	0	NULL	Differential expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential expression of epidermal growth factor receptor in juvenile and adult-onset recurrent respiratory papillomatosis .
	manualset3
247427	2	426387	16	NULL	NULL	0	NULL	epidermal growth factor receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential expression of epidermal growth factor receptor in juvenile and adult-onset recurrent respiratory papillomatosis .
	manualset3
247428	3	426387	16	NULL	NULL	0	NULL	juvenile onset recurrent respiratory papillomatosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential expression of epidermal growth factor receptor in juvenile and adult-onset recurrent respiratory papillomatosis .
	manualset3
247429	4	426387	16	NULL	NULL	0	NULL	adult-onset recurrent respiratory papillomatosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential expression of epidermal growth factor receptor in juvenile and adult-onset recurrent respiratory papillomatosis .
	manualset3
247589	1	426388	16	NULL	NULL	0	NULL	Differential expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential expression of thymus and activation regulated chemokine and its receptor CCR4 in nodal and cutaneous anaplastic large-cell lymphomas and Hodgkin 's disease .
	manualset3
247590	2	426388	16	NULL	NULL	0	NULL	thymus and activation regulated chemokine	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential expression of thymus and activation regulated chemokine and its receptor CCR4 in nodal and cutaneous anaplastic large-cell lymphomas and Hodgkin 's disease .
	manualset3
247591	3	426388	16	NULL	NULL	0	NULL	receptor CCR4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential expression of thymus and activation regulated chemokine and its receptor CCR4 in nodal and cutaneous anaplastic large-cell lymphomas and Hodgkin 's disease .
	manualset3
247592	4	426388	16	NULL	NULL	0	NULL	nodal anaplastic large-cell lymphomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential expression of thymus and activation regulated chemokine and its receptor CCR4 in nodal and cutaneous anaplastic large-cell lymphomas and Hodgkin 's disease .
	manualset3
247593	5	426388	16	NULL	NULL	0	NULL	cutaneous anaplastic large-cell lymphomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential expression of thymus and activation regulated chemokine and its receptor CCR4 in nodal and cutaneous anaplastic large-cell lymphomas and Hodgkin 's disease .
	manualset3
247594	6	426388	16	NULL	NULL	0	NULL	Hodgkin 's disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential expression of thymus and activation regulated chemokine and its receptor CCR4 in nodal and cutaneous anaplastic large-cell lymphomas and Hodgkin 's disease .
	manualset3
247430	1	426389	16	NULL	NULL	0	NULL	Objective determination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Objective determination of the hearing threshold by the Niemeyer and Sesterhenn methods ) .
	manualset3
247431	2	426389	16	NULL	NULL	0	NULL	 hearing threshold	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Objective determination of the hearing threshold by the Niemeyer and Sesterhenn methods ) .
	manualset3
247432	3	426389	16	NULL	NULL	0	NULL	Niemeyer and Sesterhenn methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Objective determination of the hearing threshold by the Niemeyer and Sesterhenn methods ) .
	manualset3
247433	1	426390	16	NULL	NULL	0	NULL	Differential immunostimulatory effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential immunostimulatory effects of Gram-positive bacteria due to their lipoteichoic acids .
	manualset3
247434	2	426390	16	NULL	NULL	0	NULL	Gram-positive bacteria 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential immunostimulatory effects of Gram-positive bacteria due to their lipoteichoic acids .
	manualset3
247436	3	426390	16	NULL	NULL	0	NULL	lipoteichoic acids	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential immunostimulatory effects of Gram-positive bacteria due to their lipoteichoic acids .
	manualset3
247372	1	426391	16	NULL	NULL	NULL	NULL	Differential influence	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differential influence of a selective melanocortin MC4 receptor antagonist ( HS014 ) on melanocortin-induced behavioral effects in rats .
	manualset3
247375	2	426391	16	NULL	NULL	0	NULL	selective melanocortin MC4 receptor antagonist ( HS014 )	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential influence of a selective melanocortin MC4 receptor antagonist ( HS014 ) on melanocortin-induced behavioral effects in rats .
	manualset3
247376	3	426391	16	NULL	NULL	0	NULL	melanocortin-induced behavioral effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential influence of a selective melanocortin MC4 receptor antagonist ( HS014 ) on melanocortin-induced behavioral effects in rats .
	manualset3
247377	4	426391	16	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential influence of a selective melanocortin MC4 receptor antagonist ( HS014 ) on melanocortin-induced behavioral effects in rats .
	manualset3
247380	1	426392	16	NULL	NULL	0	NULL	Differential proteome analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential proteome analysis of colon carcinoma cell line SW480 after reconstitution of the tumor suppressor Smad4 .
	manualset3
247389	2	426392	16	NULL	NULL	0	NULL	colon carcinoma cell line SW480	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential proteome analysis of colon carcinoma cell line SW480 after reconstitution of the tumor suppressor Smad4 .
	manualset3
247392	3	426392	16	NULL	NULL	0	NULL	reconstitution	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential proteome analysis of colon carcinoma cell line SW480 after reconstitution of the tumor suppressor Smad4 .
	manualset3
247394	4	426392	16	NULL	NULL	0	NULL	tumor suppressor Smad4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential proteome analysis of colon carcinoma cell line SW480 after reconstitution of the tumor suppressor Smad4 .
	manualset3
247398	1	426393	16	NULL	NULL	0	NULL	Differential sensitivity to bradykinin	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential sensitivity to bradykinin of esophageal distension-sensitive mechanoreceptors in vagal and sympathetic afferents of the opossum .
	manualset3
247399	2	426393	16	NULL	NULL	0	NULL	esophageal distension-sensitive mechanoreceptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential sensitivity to bradykinin of esophageal distension-sensitive mechanoreceptors in vagal and sympathetic afferents of the opossum .
	manualset3
247401	3	426393	16	NULL	NULL	0	NULL	vagal afferents	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential sensitivity to bradykinin of esophageal distension-sensitive mechanoreceptors in vagal and sympathetic afferents of the opossum .
	manualset3
247402	4	426393	16	NULL	NULL	0	NULL	sympathetic afferents	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential sensitivity to bradykinin of esophageal distension-sensitive mechanoreceptors in vagal and sympathetic afferents of the opossum .
	manualset3
247403	5	426393	16	NULL	NULL	0	NULL	opossum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential sensitivity to bradykinin of esophageal distension-sensitive mechanoreceptors in vagal and sympathetic afferents of the opossum .
	manualset3
247404	1	426394	16	NULL	NULL	NULL	NULL	Differential structure	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differential structure of the intronic promoter of the Bombyx mori A3 actin gene correlated with silkworm sensitivity/resistance to nucleopolyhedrovirus .
	manualset3
247405	2	426394	16	NULL	NULL	0	NULL	intronic promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential structure of the intronic promoter of the Bombyx mori A3 actin gene correlated with silkworm sensitivity/resistance to nucleopolyhedrovirus .
	manualset3
247406	3	426394	16	NULL	NULL	NULL	NULL	Bombyx mori A3 actin gene	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differential structure of the intronic promoter of the Bombyx mori A3 actin gene correlated with silkworm sensitivity/resistance to nucleopolyhedrovirus .
	manualset3
247423	4	426394	16	NULL	NULL	0	NULL	silkworm	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential structure of the intronic promoter of the Bombyx mori A3 actin gene correlated with silkworm sensitivity/resistance to nucleopolyhedrovirus .
	manualset3
247424	5	426394	16	NULL	NULL	0	NULL	sensitivity to nucleopolyhedrovirus	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential structure of the intronic promoter of the Bombyx mori A3 actin gene correlated with silkworm sensitivity/resistance to nucleopolyhedrovirus .
	manualset3
247425	6	426394	16	NULL	NULL	0	NULL	resistance to nucleopolyhedrovirus	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Differential structure of the intronic promoter of the Bombyx mori A3 actin gene correlated with silkworm sensitivity/resistance to nucleopolyhedrovirus .
	manualset3
247435	1	426395	16	NULL	NULL	0	NULL	Differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Differentiation of human variant small cell lung cancer cell lines to a classic morphology by retinoic acid .
	manualset3
247437	2	426395	16	NULL	NULL	0	NULL	human variant small cell lung cancer cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Differentiation of human variant small cell lung cancer cell lines to a classic morphology by retinoic acid .
	manualset3
247438	3	426395	16	NULL	NULL	NULL	NULL	classic morphology	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differentiation of human variant small cell lung cancer cell lines to a classic morphology by retinoic acid .
	manualset3
247439	4	426395	16	NULL	NULL	0	NULL	retinoic acid	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Differentiation of human variant small cell lung cancer cell lines to a classic morphology by retinoic acid .
	manualset3
247440	1	426396	16	NULL	NULL	NULL	NULL	Differentiation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differentiation of medically important Euro-Asian tick species Ixodes ricinus , Ixodes persulcatus , Ixodes hexagonus , and Dermacentor reticulatus by polymerase chain reaction .
	manualset3
247441	2	426396	16	NULL	NULL	0	NULL	Euro-Asian tick species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Differentiation of medically important Euro-Asian tick species Ixodes ricinus , Ixodes persulcatus , Ixodes hexagonus , and Dermacentor reticulatus by polymerase chain reaction .
	manualset3
247442	3	426396	16	NULL	NULL	0	NULL	Ixodes ricinus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Differentiation of medically important Euro-Asian tick species Ixodes ricinus , Ixodes persulcatus , Ixodes hexagonus , and Dermacentor reticulatus by polymerase chain reaction .
	manualset3
247443	4	426396	16	NULL	NULL	0	NULL	Ixodes persulcatus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Differentiation of medically important Euro-Asian tick species Ixodes ricinus , Ixodes persulcatus , Ixodes hexagonus , and Dermacentor reticulatus by polymerase chain reaction .
	manualset3
247444	5	426396	16	NULL	NULL	0	NULL	Ixodes hexagonus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Differentiation of medically important Euro-Asian tick species Ixodes ricinus , Ixodes persulcatus , Ixodes hexagonus , and Dermacentor reticulatus by polymerase chain reaction .
	manualset3
247445	6	426396	16	NULL	NULL	0	NULL	Dermacentor reticulatus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Differentiation of medically important Euro-Asian tick species Ixodes ricinus , Ixodes persulcatus , Ixodes hexagonus , and Dermacentor reticulatus by polymerase chain reaction .
	manualset3
247446	7	426396	16	NULL	NULL	0	NULL	polymerase chain reaction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Differentiation of medically important Euro-Asian tick species Ixodes ricinus , Ixodes persulcatus , Ixodes hexagonus , and Dermacentor reticulatus by polymerase chain reaction .
	manualset3
247447	1	426397	16	NULL	NULL	NULL	NULL	Differentiation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differentiation was assessed using morphological criteria and the level of plasminogen activator activity .
	manualset3
247448	2	426397	16	NULL	NULL	0	NULL	morphological criteria	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Differentiation was assessed using morphological criteria and the level of plasminogen activator activity .
	manualset3
247449	3	426397	16	NULL	NULL	0	NULL	level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Differentiation was assessed using morphological criteria and the level of plasminogen activator activity .
	manualset3
247450	4	426397	16	NULL	NULL	0	NULL	plasminogen activator activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Differentiation was assessed using morphological criteria and the level of plasminogen activator activity .
	manualset3
247457	1	426398	16	NULL	NULL	0	NULL	Differing patterns	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Differing patterns of membrane sialylation may have contributed to the contrasting hepatic tumorigenicities of LD and CD cells ; beta-galactoside alpha 2 , 6-sialyltransferase mRNA levels and activity were approximately four-fold higher in LD than CD cells and qualitative and quantitative differences existed between their ganglioside profiles .
	manualset3
247458	2	426398	16	NULL	NULL	0	NULL	membrane sialylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Differing patterns of membrane sialylation may have contributed to the contrasting hepatic tumorigenicities of LD and CD cells ; beta-galactoside alpha 2 , 6-sialyltransferase mRNA levels and activity were approximately four-fold higher in LD than CD cells and qualitative and quantitative differences existed between their ganglioside profiles .
	manualset3
247459	3	426398	16	NULL	NULL	0	NULL	hepatic tumorigenicities	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Differing patterns of membrane sialylation may have contributed to the contrasting hepatic tumorigenicities of LD and CD cells ; beta-galactoside alpha 2 , 6-sialyltransferase mRNA levels and activity were approximately four-fold higher in LD than CD cells and qualitative and quantitative differences existed between their ganglioside profiles .
	manualset3
247460	4	426398	16	NULL	NULL	0	NULL	LD cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Differing patterns of membrane sialylation may have contributed to the contrasting hepatic tumorigenicities of LD and CD cells ; beta-galactoside alpha 2 , 6-sialyltransferase mRNA levels and activity were approximately four-fold higher in LD than CD cells and qualitative and quantitative differences existed between their ganglioside profiles .
	manualset3
247461	5	426398	16	NULL	NULL	0	NULL	CD cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Differing patterns of membrane sialylation may have contributed to the contrasting hepatic tumorigenicities of LD and CD cells ; beta-galactoside alpha 2 , 6-sialyltransferase mRNA levels and activity were approximately four-fold higher in LD than CD cells and qualitative and quantitative differences existed between their ganglioside profiles .
	manualset3
247595	6	426398	16	NULL	NULL	NULL	NULL	beta-galactoside alpha 2 , 6-sialyltransferase mRNA levels	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differing patterns of membrane sialylation may have contributed to the contrasting hepatic tumorigenicities of LD and CD cells ; beta-galactoside alpha 2 , 6-sialyltransferase mRNA levels and activity were approximately four-fold higher in LD than CD cells and qualitative and quantitative differences existed between their ganglioside profiles .
	manualset3
247596	7	426398	16	NULL	NULL	0	NULL	beta-galactoside alpha 2 , 6-sialyltransferase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Differing patterns of membrane sialylation may have contributed to the contrasting hepatic tumorigenicities of LD and CD cells ; beta-galactoside alpha 2 , 6-sialyltransferase mRNA levels and activity were approximately four-fold higher in LD than CD cells and qualitative and quantitative differences existed between their ganglioside profiles .
	manualset3
247597	8	426398	16	NULL	NULL	NULL	NULL	four-fold	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Differing patterns of membrane sialylation may have contributed to the contrasting hepatic tumorigenicities of LD and CD cells ; beta-galactoside alpha 2 , 6-sialyltransferase mRNA levels and activity were approximately four-fold higher in LD than CD cells and qualitative and quantitative differences existed between their ganglioside profiles .
	manualset3
247598	9	426398	16	NULL	NULL	0	NULL	LD cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Differing patterns of membrane sialylation may have contributed to the contrasting hepatic tumorigenicities of LD and CD cells ; beta-galactoside alpha 2 , 6-sialyltransferase mRNA levels and activity were approximately four-fold higher in LD than CD cells and qualitative and quantitative differences existed between their ganglioside profiles .
	manualset3
247599	10	426398	16	NULL	NULL	0	NULL	CD cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Differing patterns of membrane sialylation may have contributed to the contrasting hepatic tumorigenicities of LD and CD cells ; beta-galactoside alpha 2 , 6-sialyltransferase mRNA levels and activity were approximately four-fold higher in LD than CD cells and qualitative and quantitative differences existed between their ganglioside profiles .
	manualset3
247600	11	426398	16	NULL	NULL	0	NULL	qualitative differences	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Differing patterns of membrane sialylation may have contributed to the contrasting hepatic tumorigenicities of LD and CD cells ; beta-galactoside alpha 2 , 6-sialyltransferase mRNA levels and activity were approximately four-fold higher in LD than CD cells and qualitative and quantitative differences existed between their ganglioside profiles .
	manualset3
247601	12	426398	16	NULL	NULL	0	NULL	quantitative differences	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Differing patterns of membrane sialylation may have contributed to the contrasting hepatic tumorigenicities of LD and CD cells ; beta-galactoside alpha 2 , 6-sialyltransferase mRNA levels and activity were approximately four-fold higher in LD than CD cells and qualitative and quantitative differences existed between their ganglioside profiles .
	manualset3
247602	13	426398	16	NULL	NULL	0	NULL	ganglioside profiles	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Differing patterns of membrane sialylation may have contributed to the contrasting hepatic tumorigenicities of LD and CD cells ; beta-galactoside alpha 2 , 6-sialyltransferase mRNA levels and activity were approximately four-fold higher in LD than CD cells and qualitative and quantitative differences existed between their ganglioside profiles .
	manualset3
247603	1	426399	16	NULL	NULL	0	NULL	Difficult airway	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Difficult airway -- can intubate , ca n't ventilate .
	manualset3
247604	1	426400	16	NULL	NULL	0	NULL	Objective measurements	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( Objective measurements of disease severity and diagnostic confirmation in atopic dermatitis and urticaria ) .
	manualset3
247605	2	426400	16	NULL	NULL	0	NULL	disease severity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Objective measurements of disease severity and diagnostic confirmation in atopic dermatitis and urticaria ) .
	manualset3
247606	3	426400	16	NULL	NULL	0	NULL	diagnostic confirmation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Objective measurements of disease severity and diagnostic confirmation in atopic dermatitis and urticaria ) .
	manualset3
247607	4	426400	16	NULL	NULL	0	NULL	atopic dermatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Objective measurements of disease severity and diagnostic confirmation in atopic dermatitis and urticaria ) .
	manualset3
247608	5	426400	16	NULL	NULL	0	NULL	urticaria	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Objective measurements of disease severity and diagnostic confirmation in atopic dermatitis and urticaria ) .
	manualset3
247609	1	426401	16	NULL	NULL	0	NULL	Difficulties	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Difficulties to develop and market new products have resulted in an internationally recognized severe shortage of drugs for MUMS and , as a consequence , in unacceptable animal suffering , loss of animal life , and financial loss to farm industry .
	manualset3
247610	2	426401	16	NULL	NULL	0	NULL	products	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Difficulties to develop and market new products have resulted in an internationally recognized severe shortage of drugs for MUMS and , as a consequence , in unacceptable animal suffering , loss of animal life , and financial loss to farm industry .
	manualset3
247611	3	426401	16	NULL	NULL	0	NULL	shortage	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Difficulties to develop and market new products have resulted in an internationally recognized severe shortage of drugs for MUMS and , as a consequence , in unacceptable animal suffering , loss of animal life , and financial loss to farm industry .
	manualset3
247612	4	426401	16	NULL	NULL	0	NULL	drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Difficulties to develop and market new products have resulted in an internationally recognized severe shortage of drugs for MUMS and , as a consequence , in unacceptable animal suffering , loss of animal life , and financial loss to farm industry .
	manualset3
247613	5	426401	16	NULL	NULL	0	NULL	MUMS	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Difficulties to develop and market new products have resulted in an internationally recognized severe shortage of drugs for MUMS and , as a consequence , in unacceptable animal suffering , loss of animal life , and financial loss to farm industry .
	manualset3
247614	6	426401	16	NULL	NULL	NULL	NULL	consequence	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Difficulties to develop and market new products have resulted in an internationally recognized severe shortage of drugs for MUMS and , as a consequence , in unacceptable animal suffering , loss of animal life , and financial loss to farm industry .
	manualset3
252080	7	426401	16	NULL	NULL	NULL	NULL	animal suffering	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Difficulties to develop and market new products have resulted in an internationally recognized severe shortage of drugs for MUMS and , as a consequence , in unacceptable animal suffering , loss of animal life , and financial loss to farm industry .
	manualset3
252081	8	426401	16	NULL	NULL	0	NULL	loss of animal life	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Difficulties to develop and market new products have resulted in an internationally recognized severe shortage of drugs for MUMS and , as a consequence , in unacceptable animal suffering , loss of animal life , and financial loss to farm industry .
	manualset3
252082	9	426401	16	NULL	NULL	0	NULL	financial loss	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Difficulties to develop and market new products have resulted in an internationally recognized severe shortage of drugs for MUMS and , as a consequence , in unacceptable animal suffering , loss of animal life , and financial loss to farm industry .
	manualset3
252083	10	426401	16	NULL	NULL	0	NULL	farm industry	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Difficulties to develop and market new products have resulted in an internationally recognized severe shortage of drugs for MUMS and , as a consequence , in unacceptable animal suffering , loss of animal life , and financial loss to farm industry .
	manualset3
247451	1	426402	16	NULL	NULL	0	NULL	Diffuse staining	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Diffuse staining patterns of more than half the thickness of CINs and more than 10 % of carcinoma cells were scored as positive .
	manualset3
247452	2	426402	16	NULL	NULL	0	NULL	patterns	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Diffuse staining patterns of more than half the thickness of CINs and more than 10 % of carcinoma cells were scored as positive .
	manualset3
247453	3	426402	16	NULL	NULL	0	NULL	half the thickness	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Diffuse staining patterns of more than half the thickness of CINs and more than 10 % of carcinoma cells were scored as positive .
	manualset3
247454	4	426402	16	NULL	NULL	0	NULL	CINs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Diffuse staining patterns of more than half the thickness of CINs and more than 10 % of carcinoma cells were scored as positive .
	manualset3
247455	5	426402	16	NULL	NULL	0	NULL	10 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Diffuse staining patterns of more than half the thickness of CINs and more than 10 % of carcinoma cells were scored as positive .
	manualset3
247456	6	426402	16	NULL	NULL	0	NULL	carcinoma cells 	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Diffuse staining patterns of more than half the thickness of CINs and more than 10 % of carcinoma cells were scored as positive .
	manualset3
247462	1	426403	16	NULL	NULL	0	NULL	Diffuse hepatic fibrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Diffuse hepatic fibrosis with transient myeloproliferative disorders in Down syndrome .
	manualset3
247463	2	426403	16	NULL	NULL	0	NULL	transient myeloproliferative disorders	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Diffuse hepatic fibrosis with transient myeloproliferative disorders in Down syndrome .
	manualset3
247464	3	426403	16	NULL	NULL	0	NULL	Down syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Diffuse hepatic fibrosis with transient myeloproliferative disorders in Down syndrome .
	manualset3
247465	1	426404	16	NULL	NULL	0	NULL	Diffusion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Diffusion is one of the most important gas movement processes and the determination of the diffusion coefficient is a crucial step in any study .
	manualset3
247466	2	426404	16	NULL	NULL	0	NULL	gas movement processes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Diffusion is one of the most important gas movement processes and the determination of the diffusion coefficient is a crucial step in any study .
	manualset3
247467	3	426404	16	NULL	NULL	NULL	NULL	determination	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diffusion is one of the most important gas movement processes and the determination of the diffusion coefficient is a crucial step in any study .
	manualset3
247468	4	426404	16	NULL	NULL	0	NULL	diffusion coefficient	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Diffusion is one of the most important gas movement processes and the determination of the diffusion coefficient is a crucial step in any study .
	manualset3
247469	5	426404	16	NULL	NULL	0	NULL	step	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Diffusion is one of the most important gas movement processes and the determination of the diffusion coefficient is a crucial step in any study .
	manualset3
247470	6	426404	16	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Diffusion is one of the most important gas movement processes and the determination of the diffusion coefficient is a crucial step in any study .
	manualset3
247471	1	426405	16	NULL	NULL	0	NULL	Diffusion tensor imaging ( DTI )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Diffusion tensor imaging ( DTI ) by magnetic resonance imaging ( MRI ) is now used not only for delineating white matter fiber tracts , but also for assessing the histological characteristics of pathological tissues .
	manualset3
247472	2	426405	16	NULL	NULL	0	NULL	magnetic resonance imaging ( MRI ) 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Diffusion tensor imaging ( DTI ) by magnetic resonance imaging ( MRI ) is now used not only for delineating white matter fiber tracts , but also for assessing the histological characteristics of pathological tissues .
	manualset3
247473	3	426405	16	NULL	NULL	0	NULL	white matter fiber tracts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Diffusion tensor imaging ( DTI ) by magnetic resonance imaging ( MRI ) is now used not only for delineating white matter fiber tracts , but also for assessing the histological characteristics of pathological tissues .
	manualset3
247474	4	426405	16	NULL	NULL	0	NULL	histological characteristics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Diffusion tensor imaging ( DTI ) by magnetic resonance imaging ( MRI ) is now used not only for delineating white matter fiber tracts , but also for assessing the histological characteristics of pathological tissues .
	manualset3
247475	5	426405	16	NULL	NULL	0	NULL	 pathological tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Diffusion tensor imaging ( DTI ) by magnetic resonance imaging ( MRI ) is now used not only for delineating white matter fiber tracts , but also for assessing the histological characteristics of pathological tissues .
	manualset3
247623	1	426406	16	NULL	NULL	0	NULL	reductase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Digestion of the reductase purified from rabbit liver microsomes with carboxypeptidase Y ( CPY ) , but not with aminopeptidases , resulted in the abolishment of the capacities of the reductase to bind to phosphatidylcholine liposomes and to reconstitute an active NADH-cytochrome c reductase system upon mixing with cytochrome b5 .
	manualset3
247624	2	426406	16	NULL	NULL	NULL	NULL	rabbit liver microsomes	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Digestion of the reductase purified from rabbit liver microsomes with carboxypeptidase Y ( CPY ) , but not with aminopeptidases , resulted in the abolishment of the capacities of the reductase to bind to phosphatidylcholine liposomes and to reconstitute an active NADH-cytochrome c reductase system upon mixing with cytochrome b5 .
	manualset3
247625	3	426406	16	NULL	NULL	0	NULL	carboxypeptidase Y ( CPY )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Digestion of the reductase purified from rabbit liver microsomes with carboxypeptidase Y ( CPY ) , but not with aminopeptidases , resulted in the abolishment of the capacities of the reductase to bind to phosphatidylcholine liposomes and to reconstitute an active NADH-cytochrome c reductase system upon mixing with cytochrome b5 .
	manualset3
247626	4	426406	16	NULL	NULL	0	NULL	aminopeptidases	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Digestion of the reductase purified from rabbit liver microsomes with carboxypeptidase Y ( CPY ) , but not with aminopeptidases , resulted in the abolishment of the capacities of the reductase to bind to phosphatidylcholine liposomes and to reconstitute an active NADH-cytochrome c reductase system upon mixing with cytochrome b5 .
	manualset3
247627	5	426406	16	NULL	NULL	0	NULL	abolishment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Digestion of the reductase purified from rabbit liver microsomes with carboxypeptidase Y ( CPY ) , but not with aminopeptidases , resulted in the abolishment of the capacities of the reductase to bind to phosphatidylcholine liposomes and to reconstitute an active NADH-cytochrome c reductase system upon mixing with cytochrome b5 .
	manualset3
247628	6	426406	16	NULL	NULL	0	NULL	capacities	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Digestion of the reductase purified from rabbit liver microsomes with carboxypeptidase Y ( CPY ) , but not with aminopeptidases , resulted in the abolishment of the capacities of the reductase to bind to phosphatidylcholine liposomes and to reconstitute an active NADH-cytochrome c reductase system upon mixing with cytochrome b5 .
	manualset3
247629	7	426406	16	NULL	NULL	0	NULL	reductase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Digestion of the reductase purified from rabbit liver microsomes with carboxypeptidase Y ( CPY ) , but not with aminopeptidases , resulted in the abolishment of the capacities of the reductase to bind to phosphatidylcholine liposomes and to reconstitute an active NADH-cytochrome c reductase system upon mixing with cytochrome b5 .
	manualset3
247630	8	426406	16	NULL	NULL	0	NULL	phosphatidylcholine liposomes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Digestion of the reductase purified from rabbit liver microsomes with carboxypeptidase Y ( CPY ) , but not with aminopeptidases , resulted in the abolishment of the capacities of the reductase to bind to phosphatidylcholine liposomes and to reconstitute an active NADH-cytochrome c reductase system upon mixing with cytochrome b5 .
	manualset3
247631	9	426406	16	NULL	NULL	0	NULL	active NADH-cytochrome c reductase system	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Digestion of the reductase purified from rabbit liver microsomes with carboxypeptidase Y ( CPY ) , but not with aminopeptidases , resulted in the abolishment of the capacities of the reductase to bind to phosphatidylcholine liposomes and to reconstitute an active NADH-cytochrome c reductase system upon mixing with cytochrome b5 .
	manualset3
247632	10	426406	16	NULL	NULL	0	NULL	cytochrome b5	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Digestion of the reductase purified from rabbit liver microsomes with carboxypeptidase Y ( CPY ) , but not with aminopeptidases , resulted in the abolishment of the capacities of the reductase to bind to phosphatidylcholine liposomes and to reconstitute an active NADH-cytochrome c reductase system upon mixing with cytochrome b5 .
	manualset3
247633	11	426406	16	NULL	NULL	0	NULL	Digestion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Digestion of the reductase purified from rabbit liver microsomes with carboxypeptidase Y ( CPY ) , but not with aminopeptidases , resulted in the abolishment of the capacities of the reductase to bind to phosphatidylcholine liposomes and to reconstitute an active NADH-cytochrome c reductase system upon mixing with cytochrome b5 .
	manualset3
247634	1	426407	16	NULL	NULL	0	NULL	Digital subtraction angiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Digital subtraction angiography later showed fibromuscular dysplasia of both carotid artery systems .
	manualset3
247635	2	426407	16	NULL	NULL	0	NULL	fibromuscular dysplasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Digital subtraction angiography later showed fibromuscular dysplasia of both carotid artery systems .
	manualset3
247636	3	426407	16	NULL	NULL	0	NULL	carotid artery systems	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Digital subtraction angiography later showed fibromuscular dysplasia of both carotid artery systems .
	manualset3
247637	1	426408	16	NULL	NULL	0	NULL	Observation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Observation on two cases of anemia due to falciform hemathies ) .
	manualset3
247638	2	426408	16	NULL	NULL	0	NULL	two cases	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Observation on two cases of anemia due to falciform hemathies ) .
	manualset3
247639	3	426408	16	NULL	NULL	0	NULL	anemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Observation on two cases of anemia due to falciform hemathies ) .
	manualset3
247640	4	426408	16	NULL	NULL	0	NULL	falciform hemathies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Observation on two cases of anemia due to falciform hemathies ) .
	manualset3
247641	1	426409	16	NULL	NULL	0	NULL	Digitoxin	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Digitoxin and ouabain were equipotent ; however , digoxin was significantly less potent .
	manualset3
247642	2	426409	16	NULL	NULL	0	NULL	ouabain	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Digitoxin and ouabain were equipotent ; however , digoxin was significantly less potent .
	manualset3
247643	3	426409	16	NULL	NULL	0	NULL	digoxin	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Digitoxin and ouabain were equipotent ; however , digoxin was significantly less potent .
	manualset3
247644	1	426410	16	NULL	NULL	0	NULL	Dihydroceramide desaturase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Dihydroceramide desaturase is responsible for the introduction of the 4 , 5-trans double bond into ceramide .
	manualset3
247645	2	426410	16	NULL	NULL	NULL	NULL	introduction	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dihydroceramide desaturase is responsible for the introduction of the 4 , 5-trans double bond into ceramide .
	manualset3
247646	3	426410	16	NULL	NULL	NULL	NULL	4 , 5-trans double bond	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dihydroceramide desaturase is responsible for the introduction of the 4 , 5-trans double bond into ceramide .
	manualset3
258599	4	426410	16	NULL	NULL	NULL	NULL	ceramide	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dihydroceramide desaturase is responsible for the introduction of the 4 , 5-trans double bond into ceramide .
	manualset3
247647	1	426411	16	NULL	NULL	0	NULL	Diisocyanates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Diisocyanates are chemically reactive and induce asthma , but data on genotoxic effects of diisocyanates in humans are limited .
	manualset3
247648	2	426411	16	NULL	NULL	0	NULL	asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Diisocyanates are chemically reactive and induce asthma , but data on genotoxic effects of diisocyanates in humans are limited .
	manualset3
247649	3	426411	16	NULL	NULL	0	NULL	data	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Diisocyanates are chemically reactive and induce asthma , but data on genotoxic effects of diisocyanates in humans are limited .
	manualset3
247650	4	426411	16	NULL	NULL	0	NULL	genotoxic effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Diisocyanates are chemically reactive and induce asthma , but data on genotoxic effects of diisocyanates in humans are limited .
	manualset3
247651	5	426411	16	NULL	NULL	0	NULL	diisocyanates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Diisocyanates are chemically reactive and induce asthma , but data on genotoxic effects of diisocyanates in humans are limited .
	manualset3
247652	6	426411	16	NULL	NULL	0	NULL	humans	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Diisocyanates are chemically reactive and induce asthma , but data on genotoxic effects of diisocyanates in humans are limited .
	manualset3
247653	1	426412	16	NULL	NULL	NULL	NULL	Dilemmas	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dilemmas in managing intracerebral hemorrhage and thromboembolism .
	manualset3
247654	2	426412	16	NULL	NULL	0	NULL	intracerebral hemorrhage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dilemmas in managing intracerebral hemorrhage and thromboembolism .
	manualset3
247655	3	426412	16	NULL	NULL	0	NULL	thromboembolism	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dilemmas in managing intracerebral hemorrhage and thromboembolism .
	manualset3
247656	1	426413	16	NULL	NULL	0	NULL	Dimethyl 2 - ( amino-methyl-ene ) malonate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Dimethyl 2 - ( amino-methyl-ene ) malonate .
	manualset3
247658	1	426414	16	NULL	NULL	0	NULL	Diphenylamine metabolism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Diphenylamine metabolism and ethylene action were evaluated as factors influencing the development of ` Braeburn ' apple internal browning and cavitation during cold storage .
	manualset3
247659	2	426414	16	NULL	NULL	0	NULL	ethylene action	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Diphenylamine metabolism and ethylene action were evaluated as factors influencing the development of ` Braeburn ' apple internal browning and cavitation during cold storage .
	manualset3
247660	3	426414	16	NULL	NULL	0	NULL	factors	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Diphenylamine metabolism and ethylene action were evaluated as factors influencing the development of ` Braeburn ' apple internal browning and cavitation during cold storage .
	manualset3
247661	4	426414	16	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Diphenylamine metabolism and ethylene action were evaluated as factors influencing the development of ` Braeburn ' apple internal browning and cavitation during cold storage .
	manualset3
247662	5	426414	16	NULL	NULL	0	NULL	Braeburn ' apple	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Diphenylamine metabolism and ethylene action were evaluated as factors influencing the development of ` Braeburn ' apple internal browning and cavitation during cold storage .
	manualset3
247663	6	426414	16	NULL	NULL	NULL	NULL	internal browning	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diphenylamine metabolism and ethylene action were evaluated as factors influencing the development of ` Braeburn ' apple internal browning and cavitation during cold storage .
	manualset3
247664	7	426414	16	NULL	NULL	0	NULL	cavitation	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Diphenylamine metabolism and ethylene action were evaluated as factors influencing the development of ` Braeburn ' apple internal browning and cavitation during cold storage .
	manualset3
247665	8	426414	16	NULL	NULL	0	NULL	cold storage	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Diphenylamine metabolism and ethylene action were evaluated as factors influencing the development of ` Braeburn ' apple internal browning and cavitation during cold storage .
	manualset3
247666	1	426415	16	NULL	NULL	0	NULL	Diphosphonates	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Diphosphonates are potent inhibitors of bone resorption , they have been evaluated in several clinical trials for bone metastases .
	manualset3
247667	2	426415	16	NULL	NULL	NULL	NULL	potent inhibitors	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diphosphonates are potent inhibitors of bone resorption , they have been evaluated in several clinical trials for bone metastases .
	manualset3
247668	3	426415	16	NULL	NULL	0	NULL	bone resorption	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Diphosphonates are potent inhibitors of bone resorption , they have been evaluated in several clinical trials for bone metastases .
	manualset3
247669	4	426415	16	NULL	NULL	0	NULL	clinical trials	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Diphosphonates are potent inhibitors of bone resorption , they have been evaluated in several clinical trials for bone metastases .
	manualset3
247670	5	426415	16	NULL	NULL	0	NULL	bone metastases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Diphosphonates are potent inhibitors of bone resorption , they have been evaluated in several clinical trials for bone metastases .
	manualset3
247671	1	426416	16	NULL	NULL	0	NULL	Diplopia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Diplopia developed after the dose of carbamazepine was increased to 700 mg/day .
	manualset3
247672	2	426416	16	NULL	NULL	0	NULL	dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Diplopia developed after the dose of carbamazepine was increased to 700 mg/day .
	manualset3
247673	3	426416	16	NULL	NULL	0	NULL	carbamazepine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Diplopia developed after the dose of carbamazepine was increased to 700 mg/day .
	manualset3
247674	4	426416	16	NULL	NULL	0	NULL	700 mg/day	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Diplopia developed after the dose of carbamazepine was increased to 700 mg/day .
	manualset3
247675	1	426417	16	NULL	NULL	0	NULL	Dipyridamole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Dipyridamole was found to bind extensively ( 97 % ) to rat plasma proteins , which may explain the discrepancy between the concentrations of dipyridamole required to inhibit nucleoside incorporation in vitro , in serum-free media , and those needed in vivo .
	manualset3
247676	2	426417	16	NULL	NULL	0	NULL	97 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Dipyridamole was found to bind extensively ( 97 % ) to rat plasma proteins , which may explain the discrepancy between the concentrations of dipyridamole required to inhibit nucleoside incorporation in vitro , in serum-free media , and those needed in vivo .
	manualset3
247677	3	426417	16	NULL	NULL	0	NULL	rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Dipyridamole was found to bind extensively ( 97 % ) to rat plasma proteins , which may explain the discrepancy between the concentrations of dipyridamole required to inhibit nucleoside incorporation in vitro , in serum-free media , and those needed in vivo .
	manualset3
247678	4	426417	16	NULL	NULL	0	NULL	plasma proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Dipyridamole was found to bind extensively ( 97 % ) to rat plasma proteins , which may explain the discrepancy between the concentrations of dipyridamole required to inhibit nucleoside incorporation in vitro , in serum-free media , and those needed in vivo .
	manualset3
247679	5	426417	16	NULL	NULL	0	NULL	discrepancy	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Dipyridamole was found to bind extensively ( 97 % ) to rat plasma proteins , which may explain the discrepancy between the concentrations of dipyridamole required to inhibit nucleoside incorporation in vitro , in serum-free media , and those needed in vivo .
	manualset3
247680	6	426417	16	NULL	NULL	0	NULL	concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dipyridamole was found to bind extensively ( 97 % ) to rat plasma proteins , which may explain the discrepancy between the concentrations of dipyridamole required to inhibit nucleoside incorporation in vitro , in serum-free media , and those needed in vivo .
	manualset3
247681	7	426417	16	NULL	NULL	0	NULL	dipyridamole	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Dipyridamole was found to bind extensively ( 97 % ) to rat plasma proteins , which may explain the discrepancy between the concentrations of dipyridamole required to inhibit nucleoside incorporation in vitro , in serum-free media , and those needed in vivo .
	manualset3
247682	8	426417	16	NULL	NULL	0	NULL	nucleoside incorporation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dipyridamole was found to bind extensively ( 97 % ) to rat plasma proteins , which may explain the discrepancy between the concentrations of dipyridamole required to inhibit nucleoside incorporation in vitro , in serum-free media , and those needed in vivo .
	manualset3
247683	9	426417	16	NULL	NULL	0	NULL	serum-free media	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Dipyridamole was found to bind extensively ( 97 % ) to rat plasma proteins , which may explain the discrepancy between the concentrations of dipyridamole required to inhibit nucleoside incorporation in vitro , in serum-free media , and those needed in vivo .
	manualset3
247684	1	426418	16	NULL	NULL	0	NULL	ACETYLCARNITINE	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( ACETYLCARNITINE AS AN ACETYL DONOR IN ENZYMATIC FORMATION OF ACETYLCHOLINE ) .
	manualset3
247685	2	426418	16	NULL	NULL	0	NULL	ACETYL DONOR	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( ACETYLCARNITINE AS AN ACETYL DONOR IN ENZYMATIC FORMATION OF ACETYLCHOLINE ) .
	manualset3
247686	3	426418	16	NULL	NULL	0	NULL	ENZYMATIC FORMATION	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( ACETYLCARNITINE AS AN ACETYL DONOR IN ENZYMATIC FORMATION OF ACETYLCHOLINE ) .
	manualset3
247687	4	426418	16	NULL	NULL	0	NULL	ACETYLCHOLINE	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	( ACETYLCARNITINE AS AN ACETYL DONOR IN ENZYMATIC FORMATION OF ACETYLCHOLINE ) .
	manualset3
247688	1	426419	16	NULL	NULL	NULL	NULL	Observations	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Observations of flight phobia ) .
	manualset3
247689	2	426419	16	NULL	NULL	0	NULL	flight phobia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Observations of flight phobia ) .
	manualset3
247690	1	426420	16	NULL	NULL	0	NULL	Direct C-glycosylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct C-glycosylation of indole with unprotected mono - , di - , and trisaccharides : a one-pot synthesis of 1-deoxy-1 , 1 - bis ( 3-indolyl ) alditols .
	manualset3
247691	2	426420	16	NULL	NULL	0	NULL	indole	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct C-glycosylation of indole with unprotected mono - , di - , and trisaccharides : a one-pot synthesis of 1-deoxy-1 , 1 - bis ( 3-indolyl ) alditols .
	manualset3
247692	3	426420	16	NULL	NULL	0	NULL	mono-saccharides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct C-glycosylation of indole with unprotected mono - , di - , and trisaccharides : a one-pot synthesis of 1-deoxy-1 , 1 - bis ( 3-indolyl ) alditols .
	manualset3
247693	4	426420	16	NULL	NULL	0	NULL	di -saccharides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct C-glycosylation of indole with unprotected mono - , di - , and trisaccharides : a one-pot synthesis of 1-deoxy-1 , 1 - bis ( 3-indolyl ) alditols .
	manualset3
247694	5	426420	16	NULL	NULL	0	NULL	trisaccharides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct C-glycosylation of indole with unprotected mono - , di - , and trisaccharides : a one-pot synthesis of 1-deoxy-1 , 1 - bis ( 3-indolyl ) alditols .
	manualset3
247695	6	426420	16	NULL	NULL	0	NULL	one-pot synthesis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct C-glycosylation of indole with unprotected mono - , di - , and trisaccharides : a one-pot synthesis of 1-deoxy-1 , 1 - bis ( 3-indolyl ) alditols .
	manualset3
247696	7	426420	16	NULL	NULL	0	NULL	1-deoxy-1 , 1 - bis ( 3-indolyl ) alditols	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct C-glycosylation of indole with unprotected mono - , di - , and trisaccharides : a one-pot synthesis of 1-deoxy-1 , 1 - bis ( 3-indolyl ) alditols .
	manualset3
247697	1	426421	16	NULL	NULL	0	NULL	Direct effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct and indirect effects in vaccine efficacy and effectiveness .
	manualset3
247698	2	426421	16	NULL	NULL	0	NULL	indirect effects	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct and indirect effects in vaccine efficacy and effectiveness .
	manualset3
247699	3	426421	16	NULL	NULL	0	NULL	vaccine efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct and indirect effects in vaccine efficacy and effectiveness .
	manualset3
247700	4	426421	16	NULL	NULL	0	NULL	vaccine effectiveness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct and indirect effects in vaccine efficacy and effectiveness .
	manualset3
247701	1	426422	16	NULL	NULL	0	NULL	Direct binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct binding of GATA1 to the Prx5 promoter was demonstrated using chromatin immunoprecipitation and electrophoretic mobility shift assays .
	manualset3
247702	2	426422	16	NULL	NULL	0	NULL	GATA1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct binding of GATA1 to the Prx5 promoter was demonstrated using chromatin immunoprecipitation and electrophoretic mobility shift assays .
	manualset3
247703	3	426422	16	NULL	NULL	NULL	NULL	Prx5 promoter	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Direct binding of GATA1 to the Prx5 promoter was demonstrated using chromatin immunoprecipitation and electrophoretic mobility shift assays .
	manualset3
247704	4	426422	16	NULL	NULL	0	NULL	chromatin immunoprecipitation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct binding of GATA1 to the Prx5 promoter was demonstrated using chromatin immunoprecipitation and electrophoretic mobility shift assays .
	manualset3
247705	5	426422	16	NULL	NULL	0	NULL	electrophoretic mobility shift assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct binding of GATA1 to the Prx5 promoter was demonstrated using chromatin immunoprecipitation and electrophoretic mobility shift assays .
	manualset3
247706	1	426423	16	NULL	NULL	0	NULL	comparisons	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct comparisons of cytotoxicity and lipid peroxidation induced by tBH in freshly isolated renal cells showed that the primary cultures of cells from NPX rat kidneys retained their altered susceptibility relative to cells from control rats .
	manualset3
247707	2	426423	16	NULL	NULL	NULL	NULL	cytotoxicity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Direct comparisons of cytotoxicity and lipid peroxidation induced by tBH in freshly isolated renal cells showed that the primary cultures of cells from NPX rat kidneys retained their altered susceptibility relative to cells from control rats .
	manualset3
247708	3	426423	16	NULL	NULL	0	NULL	lipid peroxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct comparisons of cytotoxicity and lipid peroxidation induced by tBH in freshly isolated renal cells showed that the primary cultures of cells from NPX rat kidneys retained their altered susceptibility relative to cells from control rats .
	manualset3
247709	4	426423	16	NULL	NULL	0	NULL	tBH	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct comparisons of cytotoxicity and lipid peroxidation induced by tBH in freshly isolated renal cells showed that the primary cultures of cells from NPX rat kidneys retained their altered susceptibility relative to cells from control rats .
	manualset3
247710	5	426423	16	NULL	NULL	0	NULL	renal cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct comparisons of cytotoxicity and lipid peroxidation induced by tBH in freshly isolated renal cells showed that the primary cultures of cells from NPX rat kidneys retained their altered susceptibility relative to cells from control rats .
	manualset3
247711	6	426423	16	NULL	NULL	0	NULL	primary cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct comparisons of cytotoxicity and lipid peroxidation induced by tBH in freshly isolated renal cells showed that the primary cultures of cells from NPX rat kidneys retained their altered susceptibility relative to cells from control rats .
	manualset3
247712	7	426423	16	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct comparisons of cytotoxicity and lipid peroxidation induced by tBH in freshly isolated renal cells showed that the primary cultures of cells from NPX rat kidneys retained their altered susceptibility relative to cells from control rats .
	manualset3
247713	8	426423	16	NULL	NULL	0	NULL	NPX rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct comparisons of cytotoxicity and lipid peroxidation induced by tBH in freshly isolated renal cells showed that the primary cultures of cells from NPX rat kidneys retained their altered susceptibility relative to cells from control rats .
	manualset3
247714	9	426423	16	NULL	NULL	0	NULL	kidneys	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct comparisons of cytotoxicity and lipid peroxidation induced by tBH in freshly isolated renal cells showed that the primary cultures of cells from NPX rat kidneys retained their altered susceptibility relative to cells from control rats .
	manualset3
247715	10	426423	16	NULL	NULL	0	NULL	altered susceptibility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct comparisons of cytotoxicity and lipid peroxidation induced by tBH in freshly isolated renal cells showed that the primary cultures of cells from NPX rat kidneys retained their altered susceptibility relative to cells from control rats .
	manualset3
247716	11	426423	16	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct comparisons of cytotoxicity and lipid peroxidation induced by tBH in freshly isolated renal cells showed that the primary cultures of cells from NPX rat kidneys retained their altered susceptibility relative to cells from control rats .
	manualset3
247717	12	426423	16	NULL	NULL	0	NULL	control rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct comparisons of cytotoxicity and lipid peroxidation induced by tBH in freshly isolated renal cells showed that the primary cultures of cells from NPX rat kidneys retained their altered susceptibility relative to cells from control rats .
	manualset3
247718	1	426424	16	NULL	NULL	0	NULL	Direct decision making	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct decision making vs. oblique decision making : which is right ?
	manualset3
247719	2	426424	16	NULL	NULL	0	NULL	oblique decision making	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct decision making vs. oblique decision making : which is right ?
	manualset3
247720	1	426425	16	NULL	NULL	0	NULL	effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct effects of tolbutamide and insulin on peripheral glucose uptake ; a comparative study in man .
	manualset3
247721	2	426425	16	NULL	NULL	0	NULL	tolbutamide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct effects of tolbutamide and insulin on peripheral glucose uptake ; a comparative study in man .
	manualset3
247722	3	426425	16	NULL	NULL	0	NULL	insulin	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct effects of tolbutamide and insulin on peripheral glucose uptake ; a comparative study in man .
	manualset3
247723	4	426425	16	NULL	NULL	0	NULL	peripheral glucose uptake	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct effects of tolbutamide and insulin on peripheral glucose uptake ; a comparative study in man .
	manualset3
247724	5	426425	16	NULL	NULL	0	NULL	comparative study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct effects of tolbutamide and insulin on peripheral glucose uptake ; a comparative study in man .
	manualset3
247725	6	426425	16	NULL	NULL	0	NULL	man	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct effects of tolbutamide and insulin on peripheral glucose uptake ; a comparative study in man .
	manualset3
247726	1	426426	16	NULL	NULL	0	NULL	evidence	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct evidence of the formation of an intermediate aldimine between the cofactor and the active-site lysine was obtained .
	manualset3
247727	2	426426	16	NULL	NULL	0	NULL	formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct evidence of the formation of an intermediate aldimine between the cofactor and the active-site lysine was obtained .
	manualset3
247728	3	426426	16	NULL	NULL	0	NULL	intermediate aldimine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct evidence of the formation of an intermediate aldimine between the cofactor and the active-site lysine was obtained .
	manualset3
247729	4	426426	16	NULL	NULL	0	NULL	cofactor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct evidence of the formation of an intermediate aldimine between the cofactor and the active-site lysine was obtained .
	manualset3
247730	5	426426	16	NULL	NULL	0	NULL	active-site lysine	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct evidence of the formation of an intermediate aldimine between the cofactor and the active-site lysine was obtained .
	manualset3
247731	1	426427	16	NULL	NULL	NULL	NULL	evidence	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Direct evidence of the nonuniformly canted state of the spin-flop phase induced by a magnetic field applied to Fe/Cr ( 100 ) superlattices is obtained by polarized neutron reflectometry .
	manualset3
247732	2	426427	16	NULL	NULL	0	NULL	nonuniformly canted state	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct evidence of the nonuniformly canted state of the spin-flop phase induced by a magnetic field applied to Fe/Cr ( 100 ) superlattices is obtained by polarized neutron reflectometry .
	manualset3
247733	3	426427	16	NULL	NULL	0	NULL	spin-flop phase	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct evidence of the nonuniformly canted state of the spin-flop phase induced by a magnetic field applied to Fe/Cr ( 100 ) superlattices is obtained by polarized neutron reflectometry .
	manualset3
247734	4	426427	16	NULL	NULL	0	NULL	magnetic field	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct evidence of the nonuniformly canted state of the spin-flop phase induced by a magnetic field applied to Fe/Cr ( 100 ) superlattices is obtained by polarized neutron reflectometry .
	manualset3
247735	5	426427	16	NULL	NULL	NULL	NULL	Fe/Cr ( 100 ) superlattices	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Direct evidence of the nonuniformly canted state of the spin-flop phase induced by a magnetic field applied to Fe/Cr ( 100 ) superlattices is obtained by polarized neutron reflectometry .
	manualset3
247736	6	426427	16	NULL	NULL	0	NULL	polarized neutron reflectometry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct evidence of the nonuniformly canted state of the spin-flop phase induced by a magnetic field applied to Fe/Cr ( 100 ) superlattices is obtained by polarized neutron reflectometry .
	manualset3
247737	1	426428	16	NULL	NULL	0	NULL	Direct injection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct injection of a small plasma volume into the thermospray liquid chromatography-mass spectrometry system could be used to monitor drug plasma levels during a toxicity study in dogs .
	manualset3
247738	2	426428	16	NULL	NULL	0	NULL	small plasma volume	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct injection of a small plasma volume into the thermospray liquid chromatography-mass spectrometry system could be used to monitor drug plasma levels during a toxicity study in dogs .
	manualset3
247739	3	426428	16	NULL	NULL	0	NULL	thermospray liquid chromatography-mass spectrometry system	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct injection of a small plasma volume into the thermospray liquid chromatography-mass spectrometry system could be used to monitor drug plasma levels during a toxicity study in dogs .
	manualset3
247740	4	426428	16	NULL	NULL	0	NULL	drug plasma levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct injection of a small plasma volume into the thermospray liquid chromatography-mass spectrometry system could be used to monitor drug plasma levels during a toxicity study in dogs .
	manualset3
247741	5	426428	16	NULL	NULL	0	NULL	toxicity study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct injection of a small plasma volume into the thermospray liquid chromatography-mass spectrometry system could be used to monitor drug plasma levels during a toxicity study in dogs .
	manualset3
247742	6	426428	16	NULL	NULL	0	NULL	dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct injection of a small plasma volume into the thermospray liquid chromatography-mass spectrometry system could be used to monitor drug plasma levels during a toxicity study in dogs .
	manualset3
247743	1	426429	16	NULL	NULL	0	NULL	intrahepatic injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct intrahepatic injection of fibrin gel-immobilized hepatocytes is technically feasible .
	manualset3
247744	2	426429	16	NULL	NULL	0	NULL	fibrin gel	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct intrahepatic injection of fibrin gel-immobilized hepatocytes is technically feasible .
	manualset3
247745	3	426429	16	NULL	NULL	0	NULL	immobilized hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct intrahepatic injection of fibrin gel-immobilized hepatocytes is technically feasible .
	manualset3
247746	1	426430	16	NULL	NULL	0	NULL	Direct sequencing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct sequencing of the 3 ' terminus of one of these copy-back RNA species demonstrated its complementarity to the 5 ' - terminal sequence of the virus genome .
	manualset3
247747	2	426430	16	NULL	NULL	NULL	NULL	3 ' terminus	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Direct sequencing of the 3 ' terminus of one of these copy-back RNA species demonstrated its complementarity to the 5 ' - terminal sequence of the virus genome .
	manualset3
247748	3	426430	16	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct sequencing of the 3 ' terminus of one of these copy-back RNA species demonstrated its complementarity to the 5 ' - terminal sequence of the virus genome .
	manualset3
247749	4	426430	16	NULL	NULL	0	NULL	copy-back RNA species	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct sequencing of the 3 ' terminus of one of these copy-back RNA species demonstrated its complementarity to the 5 ' - terminal sequence of the virus genome .
	manualset3
247750	5	426430	16	NULL	NULL	0	NULL	complementarity	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct sequencing of the 3 ' terminus of one of these copy-back RNA species demonstrated its complementarity to the 5 ' - terminal sequence of the virus genome .
	manualset3
247751	6	426430	16	NULL	NULL	0	NULL	5 ' - terminal sequence	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct sequencing of the 3 ' terminus of one of these copy-back RNA species demonstrated its complementarity to the 5 ' - terminal sequence of the virus genome .
	manualset3
247752	7	426430	16	NULL	NULL	0	NULL	virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct sequencing of the 3 ' terminus of one of these copy-back RNA species demonstrated its complementarity to the 5 ' - terminal sequence of the virus genome .
	manualset3
247753	8	426430	16	NULL	NULL	0	NULL	genome	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct sequencing of the 3 ' terminus of one of these copy-back RNA species demonstrated its complementarity to the 5 ' - terminal sequence of the virus genome .
	manualset3
247754	1	426431	16	NULL	NULL	0	NULL	Direct visualization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct visualization of oxygen distribution in operating fuel cells .
	manualset3
247755	2	426431	16	NULL	NULL	0	NULL	oxygen distribution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct visualization of oxygen distribution in operating fuel cells .
	manualset3
247756	3	426431	16	NULL	NULL	0	NULL	operating fuel cells	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Direct visualization of oxygen distribution in operating fuel cells .
	manualset3
247757	1	426432	16	NULL	NULL	0	NULL	Directed differentiation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Directed differentiation of pES into neural lineages was induced by suspension culture in medium containing RA , SHH , and FGF combinations without going through embryoid body formation .
	manualset3
247758	2	426432	16	NULL	NULL	0	NULL	pES	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Directed differentiation of pES into neural lineages was induced by suspension culture in medium containing RA , SHH , and FGF combinations without going through embryoid body formation .
	manualset3
247759	3	426432	16	NULL	NULL	0	NULL	neural lineages	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Directed differentiation of pES into neural lineages was induced by suspension culture in medium containing RA , SHH , and FGF combinations without going through embryoid body formation .
	manualset3
247760	4	426432	16	NULL	NULL	0	NULL	suspension culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Directed differentiation of pES into neural lineages was induced by suspension culture in medium containing RA , SHH , and FGF combinations without going through embryoid body formation .
	manualset3
247761	5	426432	16	NULL	NULL	0	NULL	medium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Directed differentiation of pES into neural lineages was induced by suspension culture in medium containing RA , SHH , and FGF combinations without going through embryoid body formation .
	manualset3
247762	6	426432	16	NULL	NULL	0	NULL	RA	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Directed differentiation of pES into neural lineages was induced by suspension culture in medium containing RA , SHH , and FGF combinations without going through embryoid body formation .
	manualset3
247763	7	426432	16	NULL	NULL	0	NULL	SHH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Directed differentiation of pES into neural lineages was induced by suspension culture in medium containing RA , SHH , and FGF combinations without going through embryoid body formation .
	manualset3
247764	8	426432	16	NULL	NULL	0	NULL	FGF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Directed differentiation of pES into neural lineages was induced by suspension culture in medium containing RA , SHH , and FGF combinations without going through embryoid body formation .
	manualset3
247765	9	426432	16	NULL	NULL	0	NULL	combinations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Directed differentiation of pES into neural lineages was induced by suspension culture in medium containing RA , SHH , and FGF combinations without going through embryoid body formation .
	manualset3
247766	10	426432	16	NULL	NULL	0	NULL	embryoid body formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Directed differentiation of pES into neural lineages was induced by suspension culture in medium containing RA , SHH , and FGF combinations without going through embryoid body formation .
	manualset3
247767	1	426433	16	NULL	NULL	0	NULL	Directed prescription	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Directed prescription of azathioprine dependent on phenotypic expression of the thiopurine methyltransferase gene is now accepted practice .
	manualset3
247768	2	426433	16	NULL	NULL	0	NULL	azathioprine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Directed prescription of azathioprine dependent on phenotypic expression of the thiopurine methyltransferase gene is now accepted practice .
	manualset3
247769	3	426433	16	NULL	NULL	0	NULL	phenotypic expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Directed prescription of azathioprine dependent on phenotypic expression of the thiopurine methyltransferase gene is now accepted practice .
	manualset3
247770	4	426433	16	NULL	NULL	0	NULL	thiopurine methyltransferase gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Directed prescription of azathioprine dependent on phenotypic expression of the thiopurine methyltransferase gene is now accepted practice .
	manualset3
247771	5	426433	16	NULL	NULL	0	NULL	practice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Directed prescription of azathioprine dependent on phenotypic expression of the thiopurine methyltransferase gene is now accepted practice .
	manualset3
247772	1	426434	16	NULL	NULL	0	NULL	Directing differentiation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Directing differentiation of human embryonic stem cells ( hESCs ) into specific cell types using an easy and reproducible protocol is a prerequisite for the clinical use of hESCs in regenerative-medicine procedures .
	manualset3
247773	2	426434	16	NULL	NULL	0	NULL	human embryonic stem cells ( hESCs )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Directing differentiation of human embryonic stem cells ( hESCs ) into specific cell types using an easy and reproducible protocol is a prerequisite for the clinical use of hESCs in regenerative-medicine procedures .
	manualset3
247774	3	426434	16	NULL	NULL	0	NULL	specific cell types	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Directing differentiation of human embryonic stem cells ( hESCs ) into specific cell types using an easy and reproducible protocol is a prerequisite for the clinical use of hESCs in regenerative-medicine procedures .
	manualset3
247775	4	426434	16	NULL	NULL	0	NULL	reproducible protocol	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Directing differentiation of human embryonic stem cells ( hESCs ) into specific cell types using an easy and reproducible protocol is a prerequisite for the clinical use of hESCs in regenerative-medicine procedures .
	manualset3
247776	5	426434	16	NULL	NULL	0	NULL	prerequisite	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Directing differentiation of human embryonic stem cells ( hESCs ) into specific cell types using an easy and reproducible protocol is a prerequisite for the clinical use of hESCs in regenerative-medicine procedures .
	manualset3
247777	6	426434	16	NULL	NULL	0	NULL	clinical use	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Directing differentiation of human embryonic stem cells ( hESCs ) into specific cell types using an easy and reproducible protocol is a prerequisite for the clinical use of hESCs in regenerative-medicine procedures .
	manualset3
247778	7	426434	16	NULL	NULL	0	NULL	hESCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Directing differentiation of human embryonic stem cells ( hESCs ) into specific cell types using an easy and reproducible protocol is a prerequisite for the clinical use of hESCs in regenerative-medicine procedures .
	manualset3
247779	8	426434	16	NULL	NULL	0	NULL	regenerative-medicine procedures	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Directing differentiation of human embryonic stem cells ( hESCs ) into specific cell types using an easy and reproducible protocol is a prerequisite for the clinical use of hESCs in regenerative-medicine procedures .
	manualset3
247780	1	426435	16	NULL	NULL	0	NULL	Disability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Disability and psychologic distress in patients with nonspecific and specific arm pain .
	manualset3
247781	2	426435	16	NULL	NULL	0	NULL	psychologic distress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Disability and psychologic distress in patients with nonspecific and specific arm pain .
	manualset3
247782	3	426435	16	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Disability and psychologic distress in patients with nonspecific and specific arm pain .
	manualset3
247783	4	426435	16	NULL	NULL	0	NULL	nonspecific arm pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Disability and psychologic distress in patients with nonspecific and specific arm pain .
	manualset3
247784	5	426435	16	NULL	NULL	0	NULL	specific arm pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Disability and psychologic distress in patients with nonspecific and specific arm pain .
	manualset3
247785	1	426436	16	NULL	NULL	0	NULL	Disadvantages	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Disadvantages of the procedure are related to the poor panoramic view , subjective ( operator-dependent ) interpretation and limitations related to the physics of ultrasound .
	manualset3
247786	2	426436	16	NULL	NULL	0	NULL	procedure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Disadvantages of the procedure are related to the poor panoramic view , subjective ( operator-dependent ) interpretation and limitations related to the physics of ultrasound .
	manualset3
247787	3	426436	16	NULL	NULL	0	NULL	poor panoramic view	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Disadvantages of the procedure are related to the poor panoramic view , subjective ( operator-dependent ) interpretation and limitations related to the physics of ultrasound .
	manualset3
247788	4	426436	16	NULL	NULL	0	NULL	subjective ( operator-dependent ) interpretation	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Disadvantages of the procedure are related to the poor panoramic view , subjective ( operator-dependent ) interpretation and limitations related to the physics of ultrasound .
	manualset3
247789	5	426436	16	NULL	NULL	0	NULL	limitations	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Disadvantages of the procedure are related to the poor panoramic view , subjective ( operator-dependent ) interpretation and limitations related to the physics of ultrasound .
	manualset3
247790	6	426436	16	NULL	NULL	0	NULL	physics	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Disadvantages of the procedure are related to the poor panoramic view , subjective ( operator-dependent ) interpretation and limitations related to the physics of ultrasound .
	manualset3
247791	7	426436	16	NULL	NULL	0	NULL	ultrasound	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Disadvantages of the procedure are related to the poor panoramic view , subjective ( operator-dependent ) interpretation and limitations related to the physics of ultrasound .
	manualset3
247792	1	426437	16	NULL	NULL	0	NULL	Disaster planning	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Disaster planning , one of the 15 essential components of the Emergency Medical Service System Act of 1973 , should be the culmination of the establishment of other components .
	manualset3
247793	2	426437	16	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Disaster planning , one of the 15 essential components of the Emergency Medical Service System Act of 1973 , should be the culmination of the establishment of other components .
	manualset3
247794	3	426437	16	NULL	NULL	0	NULL	15 essential components	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Disaster planning , one of the 15 essential components of the Emergency Medical Service System Act of 1973 , should be the culmination of the establishment of other components .
	manualset3
247795	4	426437	16	NULL	NULL	0	NULL	Emergency Medical Service System Act of 1973	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Disaster planning , one of the 15 essential components of the Emergency Medical Service System Act of 1973 , should be the culmination of the establishment of other components .
	manualset3
247796	5	426437	16	NULL	NULL	0	NULL	culmination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Disaster planning , one of the 15 essential components of the Emergency Medical Service System Act of 1973 , should be the culmination of the establishment of other components .
	manualset3
247797	6	426437	16	NULL	NULL	0	NULL	establishment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Disaster planning , one of the 15 essential components of the Emergency Medical Service System Act of 1973 , should be the culmination of the establishment of other components .
	manualset3
247798	7	426437	16	NULL	NULL	0	NULL	components	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Disaster planning , one of the 15 essential components of the Emergency Medical Service System Act of 1973 , should be the culmination of the establishment of other components .
	manualset3
248085	1	426438	16	NULL	NULL	0	NULL	Discovery	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Discovery of 4 , 6-bis-anilino-1H-pyrrolo ( 2 , 3-d ) pyrimidines : potent inhibitors of the IGF-1R receptor tyrosine kinase .
	manualset3
248087	2	426438	16	NULL	NULL	0	NULL	4 , 6-bis-anilino-1H-pyrrolo ( 2 , 3-d ) pyrimidines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Discovery of 4 , 6-bis-anilino-1H-pyrrolo ( 2 , 3-d ) pyrimidines : potent inhibitors of the IGF-1R receptor tyrosine kinase .
	manualset3
248093	3	426438	16	NULL	NULL	0	NULL	potent inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Discovery of 4 , 6-bis-anilino-1H-pyrrolo ( 2 , 3-d ) pyrimidines : potent inhibitors of the IGF-1R receptor tyrosine kinase .
	manualset3
248095	4	426438	16	NULL	NULL	0	NULL	IGF-1R receptor tyrosine kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Discovery of 4 , 6-bis-anilino-1H-pyrrolo ( 2 , 3-d ) pyrimidines : potent inhibitors of the IGF-1R receptor tyrosine kinase .
	manualset3
248161	1	426439	16	NULL	NULL	0	NULL	Discovery	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Discovery of a small-molecule inhibitor of { beta } -1 , 6 - glucan synthesis .
	manualset3
248162	2	426439	16	NULL	NULL	0	NULL	small-molecule inhibitor	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Discovery of a small-molecule inhibitor of { beta } -1 , 6 - glucan synthesis .
	manualset3
248166	3	426439	16	NULL	NULL	0	NULL	{ beta } -1 , 6 - glucan synthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Discovery of a small-molecule inhibitor of { beta } -1 , 6 - glucan synthesis .
	manualset3
248169	1	426440	16	NULL	NULL	0	NULL	Discovery	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Discovery of radio emission from the brown dwarf LP944-20 .
	manualset3
248175	2	426440	16	NULL	NULL	0	NULL	radio emission	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Discovery of radio emission from the brown dwarf LP944-20 .
	manualset3
248198	3	426440	16	NULL	NULL	0	NULL	 brown dwarf LP944-20	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Discovery of radio emission from the brown dwarf LP944-20 .
	manualset3
248199	1	426441	16	NULL	NULL	0	NULL	Discrepancy	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Discrepancy between clinical symptoms and Tc-99m MDP bone scan findings before and after strontium-89 therapy for metastatic bone pain of prostate carcinoma .
	manualset3
248200	2	426441	16	NULL	NULL	0	NULL	clinical symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Discrepancy between clinical symptoms and Tc-99m MDP bone scan findings before and after strontium-89 therapy for metastatic bone pain of prostate carcinoma .
	manualset3
248201	3	426441	16	NULL	NULL	0	NULL	Tc-99m MDP bone scan findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Discrepancy between clinical symptoms and Tc-99m MDP bone scan findings before and after strontium-89 therapy for metastatic bone pain of prostate carcinoma .
	manualset3
248202	4	426441	16	NULL	NULL	0	NULL	strontium-89 therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Discrepancy between clinical symptoms and Tc-99m MDP bone scan findings before and after strontium-89 therapy for metastatic bone pain of prostate carcinoma .
	manualset3
248203	5	426441	16	NULL	NULL	0	NULL	metastatic bone pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Discrepancy between clinical symptoms and Tc-99m MDP bone scan findings before and after strontium-89 therapy for metastatic bone pain of prostate carcinoma .
	manualset3
248204	6	426441	16	NULL	NULL	0	NULL	prostate carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Discrepancy between clinical symptoms and Tc-99m MDP bone scan findings before and after strontium-89 therapy for metastatic bone pain of prostate carcinoma .
	manualset3
248205	1	426442	16	NULL	NULL	0	NULL	Discrepant results	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Discrepant results were related to motivational set and variance in test scores .
	manualset3
248206	2	426442	16	NULL	NULL	0	NULL	motivational set	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Discrepant results were related to motivational set and variance in test scores .
	manualset3
248207	3	426442	16	NULL	NULL	0	NULL	variance	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Discrepant results were related to motivational set and variance in test scores .
	manualset3
248208	4	426442	16	NULL	NULL	0	NULL	test scores	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Discrepant results were related to motivational set and variance in test scores .
	manualset3
248209	1	426443	16	NULL	NULL	0	NULL	Discrete DNA decorations of Pt nanoparticles ( PtNPs )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Discrete DNA decorations of Pt nanoparticles ( PtNPs ) are realized for the first time , which provide a valence control over the quasi-molecular self-assembly of Au-Pt bimetallic heteronanostructures with DNA as the guide .
	manualset3
248210	2	426443	16	NULL	NULL	0	NULL	first time	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Discrete DNA decorations of Pt nanoparticles ( PtNPs ) are realized for the first time , which provide a valence control over the quasi-molecular self-assembly of Au-Pt bimetallic heteronanostructures with DNA as the guide .
	manualset3
248211	3	426443	16	NULL	NULL	0	NULL	valence control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Discrete DNA decorations of Pt nanoparticles ( PtNPs ) are realized for the first time , which provide a valence control over the quasi-molecular self-assembly of Au-Pt bimetallic heteronanostructures with DNA as the guide .
	manualset3
248212	4	426443	16	NULL	NULL	0	NULL	quasi-molecular self-assembly	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Discrete DNA decorations of Pt nanoparticles ( PtNPs ) are realized for the first time , which provide a valence control over the quasi-molecular self-assembly of Au-Pt bimetallic heteronanostructures with DNA as the guide .
	manualset3
248213	5	426443	16	NULL	NULL	0	NULL	Au-Pt bimetallic heteronanostructures	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Discrete DNA decorations of Pt nanoparticles ( PtNPs ) are realized for the first time , which provide a valence control over the quasi-molecular self-assembly of Au-Pt bimetallic heteronanostructures with DNA as the guide .
	manualset3
248214	6	426443	16	NULL	NULL	0	NULL	DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Discrete DNA decorations of Pt nanoparticles ( PtNPs ) are realized for the first time , which provide a valence control over the quasi-molecular self-assembly of Au-Pt bimetallic heteronanostructures with DNA as the guide .
	manualset3
248215	7	426443	16	NULL	NULL	0	NULL	guide	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Discrete DNA decorations of Pt nanoparticles ( PtNPs ) are realized for the first time , which provide a valence control over the quasi-molecular self-assembly of Au-Pt bimetallic heteronanostructures with DNA as the guide .
	manualset3
248216	1	426444	16	NULL	NULL	0	NULL	Discriminant analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Discriminant analysis was applied to the results of 201Tl tomography and dobutamine echocardiography to classify a/dyskinetic segments as viable or non-viable .
	manualset3
248217	2	426444	16	NULL	NULL	0	NULL	results	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Discriminant analysis was applied to the results of 201Tl tomography and dobutamine echocardiography to classify a/dyskinetic segments as viable or non-viable .
	manualset3
248218	3	426444	16	NULL	NULL	0	NULL	201Tl tomography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Discriminant analysis was applied to the results of 201Tl tomography and dobutamine echocardiography to classify a/dyskinetic segments as viable or non-viable .
	manualset3
248219	4	426444	16	NULL	NULL	0	NULL	 dobutamine echocardiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Discriminant analysis was applied to the results of 201Tl tomography and dobutamine echocardiography to classify a/dyskinetic segments as viable or non-viable .
	manualset3
248220	5	426444	16	NULL	NULL	0	NULL	a/dyskinetic segments	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Discriminant analysis was applied to the results of 201Tl tomography and dobutamine echocardiography to classify a/dyskinetic segments as viable or non-viable .
	manualset3
248221	1	426445	16	NULL	NULL	0	NULL	metastases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Discriminating metastases of mucin-producing tumors in the breast from primary mucinous carcinomas is important with regard to the striking difference in prognosis of these lesions .
	manualset3
248222	2	426445	16	NULL	NULL	0	NULL	mucin-producing tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Discriminating metastases of mucin-producing tumors in the breast from primary mucinous carcinomas is important with regard to the striking difference in prognosis of these lesions .
	manualset3
248223	3	426445	16	NULL	NULL	0	NULL	breast	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Discriminating metastases of mucin-producing tumors in the breast from primary mucinous carcinomas is important with regard to the striking difference in prognosis of these lesions .
	manualset3
248224	4	426445	16	NULL	NULL	0	NULL	 primary mucinous carcinomas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Discriminating metastases of mucin-producing tumors in the breast from primary mucinous carcinomas is important with regard to the striking difference in prognosis of these lesions .
	manualset3
248225	5	426445	16	NULL	NULL	0	NULL	difference	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Discriminating metastases of mucin-producing tumors in the breast from primary mucinous carcinomas is important with regard to the striking difference in prognosis of these lesions .
	manualset3
248226	6	426445	16	NULL	NULL	0	NULL	prognosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Discriminating metastases of mucin-producing tumors in the breast from primary mucinous carcinomas is important with regard to the striking difference in prognosis of these lesions .
	manualset3
248227	7	426445	16	NULL	NULL	0	NULL	lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Discriminating metastases of mucin-producing tumors in the breast from primary mucinous carcinomas is important with regard to the striking difference in prognosis of these lesions .
	manualset3
248228	1	426446	16	NULL	NULL	0	NULL	Discrimination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Discrimination improves only slowly as more contor cycles are deformed until the point when the entire pattern is modulated , when sensitivity increases substantially .
	manualset3
248229	2	426446	16	NULL	NULL	0	NULL	contor cycles	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Discrimination improves only slowly as more contor cycles are deformed until the point when the entire pattern is modulated , when sensitivity increases substantially .
	manualset3
248230	3	426446	16	NULL	NULL	0	NULL	point	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Discrimination improves only slowly as more contor cycles are deformed until the point when the entire pattern is modulated , when sensitivity increases substantially .
	manualset3
248231	4	426446	16	NULL	NULL	0	NULL	pattern	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Discrimination improves only slowly as more contor cycles are deformed until the point when the entire pattern is modulated , when sensitivity increases substantially .
	manualset3
248232	5	426446	16	NULL	NULL	0	NULL	sensitivity	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Discrimination improves only slowly as more contor cycles are deformed until the point when the entire pattern is modulated , when sensitivity increases substantially .
	manualset3
248233	1	426447	16	NULL	NULL	0	NULL	Discussion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Discussion : To our knowledge , this is the first reported case of unilateral vocal fold palsy secondary to vitamin B12 deficiency .
	manualset3
248234	2	426447	16	NULL	NULL	0	NULL	knowledge	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Discussion : To our knowledge , this is the first reported case of unilateral vocal fold palsy secondary to vitamin B12 deficiency .
	manualset3
248235	3	426447	16	NULL	NULL	0	NULL	first	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Discussion : To our knowledge , this is the first reported case of unilateral vocal fold palsy secondary to vitamin B12 deficiency .
	manualset3
248236	4	426447	16	NULL	NULL	0	NULL	case	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Discussion : To our knowledge , this is the first reported case of unilateral vocal fold palsy secondary to vitamin B12 deficiency .
	manualset3
248237	5	426447	16	NULL	NULL	0	NULL	unilateral vocal fold palsy secondary	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Discussion : To our knowledge , this is the first reported case of unilateral vocal fold palsy secondary to vitamin B12 deficiency .
	manualset3
248238	6	426447	16	NULL	NULL	0	NULL	vitamin B12 deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Discussion : To our knowledge , this is the first reported case of unilateral vocal fold palsy secondary to vitamin B12 deficiency .
	manualset3
248239	1	426448	16	NULL	NULL	0	NULL	Discussion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Discussion : Using Listerine prior to application of lidocaine nasal spray reduces the pain and discomfort of FNL .
	manualset3
248240	2	426448	16	NULL	NULL	0	NULL	Listerine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Discussion : Using Listerine prior to application of lidocaine nasal spray reduces the pain and discomfort of FNL .
	manualset3
248241	3	426448	16	NULL	NULL	NULL	NULL	application	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Discussion : Using Listerine prior to application of lidocaine nasal spray reduces the pain and discomfort of FNL .
	manualset3
248242	4	426448	16	NULL	NULL	0	NULL	pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Discussion : Using Listerine prior to application of lidocaine nasal spray reduces the pain and discomfort of FNL .
	manualset3
248243	5	426448	16	NULL	NULL	0	NULL	discomfort	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Discussion : Using Listerine prior to application of lidocaine nasal spray reduces the pain and discomfort of FNL .
	manualset3
248244	6	426448	16	NULL	NULL	0	NULL	FNL	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Discussion : Using Listerine prior to application of lidocaine nasal spray reduces the pain and discomfort of FNL .
	manualset3
248245	1	426449	16	NULL	NULL	NULL	NULL	Occurrence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Occurrence of antibiotic-resistant and resistance-transferring in the intestinal tract of hospitalized children in relation to E. coli strains the type of ward and to chemotherapy ) .
	manualset3
248246	2	426449	16	NULL	NULL	0	NULL	antibiotic-resistant	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Occurrence of antibiotic-resistant and resistance-transferring in the intestinal tract of hospitalized children in relation to E. coli strains the type of ward and to chemotherapy ) .
	manualset3
248247	3	426449	16	NULL	NULL	0	NULL	resistance-transferring	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Occurrence of antibiotic-resistant and resistance-transferring in the intestinal tract of hospitalized children in relation to E. coli strains the type of ward and to chemotherapy ) .
	manualset3
248248	4	426449	16	NULL	NULL	0	NULL	intestinal tract	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Occurrence of antibiotic-resistant and resistance-transferring in the intestinal tract of hospitalized children in relation to E. coli strains the type of ward and to chemotherapy ) .
	manualset3
248249	5	426449	16	NULL	NULL	0	NULL	hospitalized children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Occurrence of antibiotic-resistant and resistance-transferring in the intestinal tract of hospitalized children in relation to E. coli strains the type of ward and to chemotherapy ) .
	manualset3
248250	6	426449	16	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	( Occurrence of antibiotic-resistant and resistance-transferring in the intestinal tract of hospitalized children in relation to E. coli strains the type of ward and to chemotherapy ) .
	manualset3
248251	7	426449	16	NULL	NULL	0	NULL	E. coli strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Occurrence of antibiotic-resistant and resistance-transferring in the intestinal tract of hospitalized children in relation to E. coli strains the type of ward and to chemotherapy ) .
	manualset3
248252	8	426449	16	NULL	NULL	0	NULL	type of ward	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Occurrence of antibiotic-resistant and resistance-transferring in the intestinal tract of hospitalized children in relation to E. coli strains the type of ward and to chemotherapy ) .
	manualset3
248253	9	426449	16	NULL	NULL	0	NULL	chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Occurrence of antibiotic-resistant and resistance-transferring in the intestinal tract of hospitalized children in relation to E. coli strains the type of ward and to chemotherapy ) .
	manualset3
248254	1	426450	16	NULL	NULL	0	NULL	Discussion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Discussion on the thermal conductivity enhancement of nanofluids .
	manualset3
248255	2	426450	16	NULL	NULL	0	NULL	thermal conductivity enhancement	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Discussion on the thermal conductivity enhancement of nanofluids .
	manualset3
248256	3	426450	16	NULL	NULL	0	NULL	nanofluids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Discussion on the thermal conductivity enhancement of nanofluids .
	manualset3
248257	1	426451	16	NULL	NULL	0	NULL	Disease progression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Disease progression in myeloid malignancies results from the accumulation of `` mutations '' in genes that control cellular growth and differentiation .
	manualset3
248258	2	426451	16	NULL	NULL	0	NULL	myeloid malignancies	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Disease progression in myeloid malignancies results from the accumulation of `` mutations '' in genes that control cellular growth and differentiation .
	manualset3
248259	3	426451	16	NULL	NULL	0	NULL	accumulation	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Disease progression in myeloid malignancies results from the accumulation of `` mutations '' in genes that control cellular growth and differentiation .
	manualset3
248260	4	426451	16	NULL	NULL	0	NULL	mutations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Disease progression in myeloid malignancies results from the accumulation of `` mutations '' in genes that control cellular growth and differentiation .
	manualset3
248261	5	426451	16	NULL	NULL	0	NULL	genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Disease progression in myeloid malignancies results from the accumulation of `` mutations '' in genes that control cellular growth and differentiation .
	manualset3
248262	6	426451	16	NULL	NULL	0	NULL	cellular growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Disease progression in myeloid malignancies results from the accumulation of `` mutations '' in genes that control cellular growth and differentiation .
	manualset3
248263	7	426451	16	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Disease progression in myeloid malignancies results from the accumulation of `` mutations '' in genes that control cellular growth and differentiation .
	manualset3
248264	1	426452	16	NULL	NULL	0	NULL	Disease resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Disease resistance through vaccination ; its dependence on host and pathogen genotypes for success .
	manualset3
248265	2	426452	16	NULL	NULL	0	NULL	vaccination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Disease resistance through vaccination ; its dependence on host and pathogen genotypes for success .
	manualset3
248266	3	426452	16	NULL	NULL	0	NULL	dependence	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Disease resistance through vaccination ; its dependence on host and pathogen genotypes for success .
	manualset3
248267	4	426452	16	NULL	NULL	0	NULL	host genotypes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Disease resistance through vaccination ; its dependence on host and pathogen genotypes for success .
	manualset3
248268	5	426452	16	NULL	NULL	0	NULL	pathogen genotypes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Disease resistance through vaccination ; its dependence on host and pathogen genotypes for success .
	manualset3
248269	6	426452	16	NULL	NULL	NULL	NULL	success	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Disease resistance through vaccination ; its dependence on host and pathogen genotypes for success .
	manualset3
248270	1	426453	16	NULL	NULL	0	NULL	Occurrence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Occurrence of autoimmune phenomena in persons infected with HIV .
	manualset3
248271	2	426453	16	NULL	NULL	0	NULL	autoimmune phenomena	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Occurrence of autoimmune phenomena in persons infected with HIV .
	manualset3
248272	3	426453	16	NULL	NULL	0	NULL	persons	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Occurrence of autoimmune phenomena in persons infected with HIV .
	manualset3
248273	4	426453	16	NULL	NULL	0	NULL	 infected with HIV	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Occurrence of autoimmune phenomena in persons infected with HIV .
	manualset3
248274	1	426454	16	NULL	NULL	0	NULL	Displacement	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Displacement of ( 125I ) TSH bound to fat cell membranes by both Graves ' Ig and unlabeled TSH were time and temperature dependent , with similar dissociation curves , suggesting a specific binding of Graves ' Ig to the membrane sites related to the TSH receptor in the fat cells .
	manualset3
248275	2	426454	16	NULL	NULL	0	NULL	125I	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Displacement of ( 125I ) TSH bound to fat cell membranes by both Graves ' Ig and unlabeled TSH were time and temperature dependent , with similar dissociation curves , suggesting a specific binding of Graves ' Ig to the membrane sites related to the TSH receptor in the fat cells .
	manualset3
248276	3	426454	16	NULL	NULL	0	NULL	TSH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Displacement of ( 125I ) TSH bound to fat cell membranes by both Graves ' Ig and unlabeled TSH were time and temperature dependent , with similar dissociation curves , suggesting a specific binding of Graves ' Ig to the membrane sites related to the TSH receptor in the fat cells .
	manualset3
248277	4	426454	16	NULL	NULL	NULL	NULL	fat cell membranes	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Displacement of ( 125I ) TSH bound to fat cell membranes by both Graves ' Ig and unlabeled TSH were time and temperature dependent , with similar dissociation curves , suggesting a specific binding of Graves ' Ig to the membrane sites related to the TSH receptor in the fat cells .
	manualset3
248278	5	426454	16	NULL	NULL	0	NULL	Graves ' Ig	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Displacement of ( 125I ) TSH bound to fat cell membranes by both Graves ' Ig and unlabeled TSH were time and temperature dependent , with similar dissociation curves , suggesting a specific binding of Graves ' Ig to the membrane sites related to the TSH receptor in the fat cells .
	manualset3
248279	6	426454	16	NULL	NULL	0	NULL	unlabeled TSH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Displacement of ( 125I ) TSH bound to fat cell membranes by both Graves ' Ig and unlabeled TSH were time and temperature dependent , with similar dissociation curves , suggesting a specific binding of Graves ' Ig to the membrane sites related to the TSH receptor in the fat cells .
	manualset3
248280	7	426454	16	NULL	NULL	0	NULL	time	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Displacement of ( 125I ) TSH bound to fat cell membranes by both Graves ' Ig and unlabeled TSH were time and temperature dependent , with similar dissociation curves , suggesting a specific binding of Graves ' Ig to the membrane sites related to the TSH receptor in the fat cells .
	manualset3
248281	8	426454	16	NULL	NULL	0	NULL	temperature	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Displacement of ( 125I ) TSH bound to fat cell membranes by both Graves ' Ig and unlabeled TSH were time and temperature dependent , with similar dissociation curves , suggesting a specific binding of Graves ' Ig to the membrane sites related to the TSH receptor in the fat cells .
	manualset3
248282	9	426454	16	NULL	NULL	0	NULL	dissociation curves	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Displacement of ( 125I ) TSH bound to fat cell membranes by both Graves ' Ig and unlabeled TSH were time and temperature dependent , with similar dissociation curves , suggesting a specific binding of Graves ' Ig to the membrane sites related to the TSH receptor in the fat cells .
	manualset3
248283	10	426454	16	NULL	NULL	0	NULL	specific binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Displacement of ( 125I ) TSH bound to fat cell membranes by both Graves ' Ig and unlabeled TSH were time and temperature dependent , with similar dissociation curves , suggesting a specific binding of Graves ' Ig to the membrane sites related to the TSH receptor in the fat cells .
	manualset3
248284	11	426454	16	NULL	NULL	0	NULL	Graves ' Ig	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Displacement of ( 125I ) TSH bound to fat cell membranes by both Graves ' Ig and unlabeled TSH were time and temperature dependent , with similar dissociation curves , suggesting a specific binding of Graves ' Ig to the membrane sites related to the TSH receptor in the fat cells .
	manualset3
248285	12	426454	16	NULL	NULL	0	NULL	membrane sites	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Displacement of ( 125I ) TSH bound to fat cell membranes by both Graves ' Ig and unlabeled TSH were time and temperature dependent , with similar dissociation curves , suggesting a specific binding of Graves ' Ig to the membrane sites related to the TSH receptor in the fat cells .
	manualset3
248286	13	426454	16	NULL	NULL	0	NULL	TSH receptor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Displacement of ( 125I ) TSH bound to fat cell membranes by both Graves ' Ig and unlabeled TSH were time and temperature dependent , with similar dissociation curves , suggesting a specific binding of Graves ' Ig to the membrane sites related to the TSH receptor in the fat cells .
	manualset3
248287	14	426454	16	NULL	NULL	0	NULL	fat cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Displacement of ( 125I ) TSH bound to fat cell membranes by both Graves ' Ig and unlabeled TSH were time and temperature dependent , with similar dissociation curves , suggesting a specific binding of Graves ' Ig to the membrane sites related to the TSH receptor in the fat cells .
	manualset3
248288	1	426455	16	NULL	NULL	0	NULL	Disposal	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Disposal of coal combustion residues in terrestrial systems : contamination and risk management .
	manualset3
248289	2	426455	16	NULL	NULL	0	NULL	coal combustion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Disposal of coal combustion residues in terrestrial systems : contamination and risk management .
	manualset3
248290	3	426455	16	NULL	NULL	0	NULL	residues	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Disposal of coal combustion residues in terrestrial systems : contamination and risk management .
	manualset3
248291	4	426455	16	NULL	NULL	0	NULL	terrestrial systems	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Disposal of coal combustion residues in terrestrial systems : contamination and risk management .
	manualset3
248292	5	426455	16	NULL	NULL	0	NULL	contamination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Disposal of coal combustion residues in terrestrial systems : contamination and risk management .
	manualset3
248293	6	426455	16	NULL	NULL	0	NULL	risk management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Disposal of coal combustion residues in terrestrial systems : contamination and risk management .
	manualset3
248294	1	426456	16	NULL	NULL	0	NULL	Disposition	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Disposition and metabolism of ticagrelor , a novel P2Y12 receptor antagonist , in mice , rats , and marmosets .
	manualset3
248295	2	426456	16	NULL	NULL	0	NULL	metabolism	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Disposition and metabolism of ticagrelor , a novel P2Y12 receptor antagonist , in mice , rats , and marmosets .
	manualset3
248296	3	426456	16	NULL	NULL	0	NULL	ticagrelor	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Disposition and metabolism of ticagrelor , a novel P2Y12 receptor antagonist , in mice , rats , and marmosets .
	manualset3
248297	4	426456	16	NULL	NULL	NULL	NULL	P2Y12 receptor antagonist	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Disposition and metabolism of ticagrelor , a novel P2Y12 receptor antagonist , in mice , rats , and marmosets .
	manualset3
248298	5	426456	16	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Disposition and metabolism of ticagrelor , a novel P2Y12 receptor antagonist , in mice , rats , and marmosets .
	manualset3
248299	6	426456	16	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Disposition and metabolism of ticagrelor , a novel P2Y12 receptor antagonist , in mice , rats , and marmosets .
	manualset3
248300	7	426456	16	NULL	NULL	0	NULL	marmosets	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Disposition and metabolism of ticagrelor , a novel P2Y12 receptor antagonist , in mice , rats , and marmosets .
	manualset3
248301	1	426457	16	NULL	NULL	0	NULL	Disproportionate narrowing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Disproportionate narrowing of peripheral airways and decreased static elastic recoil properties of the lung predispose infants and young children to asthma .
	manualset3
248302	2	426457	16	NULL	NULL	0	NULL	peripheral airways	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Disproportionate narrowing of peripheral airways and decreased static elastic recoil properties of the lung predispose infants and young children to asthma .
	manualset3
248303	3	426457	16	NULL	NULL	0	NULL	static elastic recoil properties	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Disproportionate narrowing of peripheral airways and decreased static elastic recoil properties of the lung predispose infants and young children to asthma .
	manualset3
248304	4	426457	16	NULL	NULL	0	NULL	lung	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Disproportionate narrowing of peripheral airways and decreased static elastic recoil properties of the lung predispose infants and young children to asthma .
	manualset3
248305	5	426457	16	NULL	NULL	0	NULL	infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Disproportionate narrowing of peripheral airways and decreased static elastic recoil properties of the lung predispose infants and young children to asthma .
	manualset3
248306	6	426457	16	NULL	NULL	0	NULL	young children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Disproportionate narrowing of peripheral airways and decreased static elastic recoil properties of the lung predispose infants and young children to asthma .
	manualset3
248307	7	426457	16	NULL	NULL	0	NULL	asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Disproportionate narrowing of peripheral airways and decreased static elastic recoil properties of the lung predispose infants and young children to asthma .
	manualset3
248308	1	426458	16	NULL	NULL	0	NULL	high titers	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Disproportionately high titers of F.D. were observed when fibrin was deposited in an extracapillary site , but mesangial fibrin deposition was not accompanied by a higher excretion of F.D. than that observed in patients in whom intraglomerular fibrin was not detected .
	manualset3
248309	2	426458	16	NULL	NULL	0	NULL	F.D.	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Disproportionately high titers of F.D. were observed when fibrin was deposited in an extracapillary site , but mesangial fibrin deposition was not accompanied by a higher excretion of F.D. than that observed in patients in whom intraglomerular fibrin was not detected .
	manualset3
248310	3	426458	16	NULL	NULL	0	NULL	fibrin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Disproportionately high titers of F.D. were observed when fibrin was deposited in an extracapillary site , but mesangial fibrin deposition was not accompanied by a higher excretion of F.D. than that observed in patients in whom intraglomerular fibrin was not detected .
	manualset3
248311	4	426458	16	NULL	NULL	0	NULL	extracapillary site	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Disproportionately high titers of F.D. were observed when fibrin was deposited in an extracapillary site , but mesangial fibrin deposition was not accompanied by a higher excretion of F.D. than that observed in patients in whom intraglomerular fibrin was not detected .
	manualset3
248312	5	426458	16	NULL	NULL	0	NULL	mesangial fibrin deposition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Disproportionately high titers of F.D. were observed when fibrin was deposited in an extracapillary site , but mesangial fibrin deposition was not accompanied by a higher excretion of F.D. than that observed in patients in whom intraglomerular fibrin was not detected .
	manualset3
248313	6	426458	16	NULL	NULL	0	NULL	higher excretion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Disproportionately high titers of F.D. were observed when fibrin was deposited in an extracapillary site , but mesangial fibrin deposition was not accompanied by a higher excretion of F.D. than that observed in patients in whom intraglomerular fibrin was not detected .
	manualset3
248314	7	426458	16	NULL	NULL	0	NULL	F.D	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Disproportionately high titers of F.D. were observed when fibrin was deposited in an extracapillary site , but mesangial fibrin deposition was not accompanied by a higher excretion of F.D. than that observed in patients in whom intraglomerular fibrin was not detected .
	manualset3
248315	8	426458	16	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Disproportionately high titers of F.D. were observed when fibrin was deposited in an extracapillary site , but mesangial fibrin deposition was not accompanied by a higher excretion of F.D. than that observed in patients in whom intraglomerular fibrin was not detected .
	manualset3
248316	9	426458	16	NULL	NULL	0	NULL	intraglomerular fibrin	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Disproportionately high titers of F.D. were observed when fibrin was deposited in an extracapillary site , but mesangial fibrin deposition was not accompanied by a higher excretion of F.D. than that observed in patients in whom intraglomerular fibrin was not detected .
	manualset3
248317	1	426459	16	NULL	NULL	0	NULL	Disruption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of Erk-dependent type I interferon induction breaks the myxoma virus species barrier .
	manualset3
248318	2	426459	16	NULL	NULL	0	NULL	Erk-dependent type I interferon induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of Erk-dependent type I interferon induction breaks the myxoma virus species barrier .
	manualset3
248319	3	426459	16	NULL	NULL	0	NULL	myxoma virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of Erk-dependent type I interferon induction breaks the myxoma virus species barrier .
	manualset3
248320	4	426459	16	NULL	NULL	0	NULL	species barrier	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of Erk-dependent type I interferon induction breaks the myxoma virus species barrier .
	manualset3
248321	1	426460	16	NULL	NULL	0	NULL	Disruption	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of actin cytoskeleton mediates loss of tensile stress induced early phenotypic modulation of vascular smooth muscle cells in organ culture .
	manualset3
248322	2	426460	16	NULL	NULL	0	NULL	actin cytoskeleton	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of actin cytoskeleton mediates loss of tensile stress induced early phenotypic modulation of vascular smooth muscle cells in organ culture .
	manualset3
248323	3	426460	16	NULL	NULL	0	NULL	loss of tensile stress	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of actin cytoskeleton mediates loss of tensile stress induced early phenotypic modulation of vascular smooth muscle cells in organ culture .
	manualset3
248324	4	426460	16	NULL	NULL	0	NULL	phenotypic modulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of actin cytoskeleton mediates loss of tensile stress induced early phenotypic modulation of vascular smooth muscle cells in organ culture .
	manualset3
248325	5	426460	16	NULL	NULL	0	NULL	vascular smooth muscle cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of actin cytoskeleton mediates loss of tensile stress induced early phenotypic modulation of vascular smooth muscle cells in organ culture .
	manualset3
248326	6	426460	16	NULL	NULL	0	NULL	organ culture	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of actin cytoskeleton mediates loss of tensile stress induced early phenotypic modulation of vascular smooth muscle cells in organ culture .
	manualset3
248327	1	426461	16	NULL	NULL	0	NULL	Disruption	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of airway epithelium in asthma pathogenesis : are protozoa responsible ?
	manualset3
248328	2	426461	16	NULL	NULL	0	NULL	airway epithelium	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of airway epithelium in asthma pathogenesis : are protozoa responsible ?
	manualset3
248329	3	426461	16	NULL	NULL	0	NULL	asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of airway epithelium in asthma pathogenesis : are protozoa responsible ?
	manualset3
248330	4	426461	16	NULL	NULL	0	NULL	pathogenesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of airway epithelium in asthma pathogenesis : are protozoa responsible ?
	manualset3
248331	5	426461	16	NULL	NULL	0	NULL	protozoa	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of airway epithelium in asthma pathogenesis : are protozoa responsible ?
	manualset3
248332	1	426462	16	NULL	NULL	0	NULL	Occurrence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Occurrence of hemolytic disease of the newborn caused by irregular antibodies ) .
	manualset3
248333	2	426462	16	NULL	NULL	0	NULL	hemolytic disease of the newborn	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Occurrence of hemolytic disease of the newborn caused by irregular antibodies ) .
	manualset3
248334	3	426462	16	NULL	NULL	0	NULL	irregular antibodies	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Occurrence of hemolytic disease of the newborn caused by irregular antibodies ) .
	manualset3
248335	1	426463	16	NULL	NULL	0	NULL	Disruption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of survivin-microtubule interactions results in loss of survivin 's anti-apoptosis function and increased caspase-3 activity , a mechanism involved in cell death , during mitosis .
	manualset3
248336	2	426463	16	NULL	NULL	0	NULL	survivin-microtubule interactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of survivin-microtubule interactions results in loss of survivin 's anti-apoptosis function and increased caspase-3 activity , a mechanism involved in cell death , during mitosis .
	manualset3
248337	3	426463	16	NULL	NULL	0	NULL	results	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of survivin-microtubule interactions results in loss of survivin 's anti-apoptosis function and increased caspase-3 activity , a mechanism involved in cell death , during mitosis .
	manualset3
248338	4	426463	16	NULL	NULL	0	NULL	loss	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of survivin-microtubule interactions results in loss of survivin 's anti-apoptosis function and increased caspase-3 activity , a mechanism involved in cell death , during mitosis .
	manualset3
248339	5	426463	16	NULL	NULL	0	NULL	survivin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of survivin-microtubule interactions results in loss of survivin 's anti-apoptosis function and increased caspase-3 activity , a mechanism involved in cell death , during mitosis .
	manualset3
248340	6	426463	16	NULL	NULL	0	NULL	anti-apoptosis function	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of survivin-microtubule interactions results in loss of survivin 's anti-apoptosis function and increased caspase-3 activity , a mechanism involved in cell death , during mitosis .
	manualset3
248341	7	426463	16	NULL	NULL	0	NULL	caspase-3 activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of survivin-microtubule interactions results in loss of survivin 's anti-apoptosis function and increased caspase-3 activity , a mechanism involved in cell death , during mitosis .
	manualset3
248342	8	426463	16	NULL	NULL	0	NULL	mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of survivin-microtubule interactions results in loss of survivin 's anti-apoptosis function and increased caspase-3 activity , a mechanism involved in cell death , during mitosis .
	manualset3
248343	9	426463	16	NULL	NULL	0	NULL	cell death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of survivin-microtubule interactions results in loss of survivin 's anti-apoptosis function and increased caspase-3 activity , a mechanism involved in cell death , during mitosis .
	manualset3
248344	10	426463	16	NULL	NULL	0	NULL	mitosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of survivin-microtubule interactions results in loss of survivin 's anti-apoptosis function and increased caspase-3 activity , a mechanism involved in cell death , during mitosis .
	manualset3
248345	1	426464	16	NULL	NULL	0	NULL	Disruption	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of the cytoskeleton with the drug dihydrocytochalasin B inhibited the cell culture induced increase in integrin expression , while treatment of cultured cells with TGF-beta resulted in increased expression of the alpha 5 beta 1 integrin .
	manualset3
248346	2	426464	16	NULL	NULL	0	NULL	cytoskeleton	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of the cytoskeleton with the drug dihydrocytochalasin B inhibited the cell culture induced increase in integrin expression , while treatment of cultured cells with TGF-beta resulted in increased expression of the alpha 5 beta 1 integrin .
	manualset3
248347	3	426464	16	NULL	NULL	0	NULL	drug dihydrocytochalasin B	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of the cytoskeleton with the drug dihydrocytochalasin B inhibited the cell culture induced increase in integrin expression , while treatment of cultured cells with TGF-beta resulted in increased expression of the alpha 5 beta 1 integrin .
	manualset3
248348	4	426464	16	NULL	NULL	0	NULL	cell culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of the cytoskeleton with the drug dihydrocytochalasin B inhibited the cell culture induced increase in integrin expression , while treatment of cultured cells with TGF-beta resulted in increased expression of the alpha 5 beta 1 integrin .
	manualset3
248349	5	426464	16	NULL	NULL	0	NULL	increase	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of the cytoskeleton with the drug dihydrocytochalasin B inhibited the cell culture induced increase in integrin expression , while treatment of cultured cells with TGF-beta resulted in increased expression of the alpha 5 beta 1 integrin .
	manualset3
248350	6	426464	16	NULL	NULL	0	NULL	integrin expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of the cytoskeleton with the drug dihydrocytochalasin B inhibited the cell culture induced increase in integrin expression , while treatment of cultured cells with TGF-beta resulted in increased expression of the alpha 5 beta 1 integrin .
	manualset3
248351	7	426464	16	NULL	NULL	0	NULL	treatment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of the cytoskeleton with the drug dihydrocytochalasin B inhibited the cell culture induced increase in integrin expression , while treatment of cultured cells with TGF-beta resulted in increased expression of the alpha 5 beta 1 integrin .
	manualset3
248352	8	426464	16	NULL	NULL	0	NULL	cultured cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of the cytoskeleton with the drug dihydrocytochalasin B inhibited the cell culture induced increase in integrin expression , while treatment of cultured cells with TGF-beta resulted in increased expression of the alpha 5 beta 1 integrin .
	manualset3
248353	9	426464	16	NULL	NULL	0	NULL	TGF-beta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of the cytoskeleton with the drug dihydrocytochalasin B inhibited the cell culture induced increase in integrin expression , while treatment of cultured cells with TGF-beta resulted in increased expression of the alpha 5 beta 1 integrin .
	manualset3
248354	10	426464	16	NULL	NULL	0	NULL	increased expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of the cytoskeleton with the drug dihydrocytochalasin B inhibited the cell culture induced increase in integrin expression , while treatment of cultured cells with TGF-beta resulted in increased expression of the alpha 5 beta 1 integrin .
	manualset3
248355	11	426464	16	NULL	NULL	0	NULL	alpha 5 beta 1 integrin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of the cytoskeleton with the drug dihydrocytochalasin B inhibited the cell culture induced increase in integrin expression , while treatment of cultured cells with TGF-beta resulted in increased expression of the alpha 5 beta 1 integrin .
	manualset3
248356	1	426465	16	NULL	NULL	0	NULL	Disruption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of the loop 's tertiary structure by Ser mutations of these Cys residues either prevented receptor assembly on the cell surface , or created receptors unable to be activated by agonists or to bind the competitive antagonist , strychnine .
	manualset3
248357	2	426465	16	NULL	NULL	0	NULL	loop	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of the loop 's tertiary structure by Ser mutations of these Cys residues either prevented receptor assembly on the cell surface , or created receptors unable to be activated by agonists or to bind the competitive antagonist , strychnine .
	manualset3
248358	3	426465	16	NULL	NULL	0	NULL	tertiary structure	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of the loop 's tertiary structure by Ser mutations of these Cys residues either prevented receptor assembly on the cell surface , or created receptors unable to be activated by agonists or to bind the competitive antagonist , strychnine .
	manualset3
248361	4	426465	16	NULL	NULL	0	NULL	Ser mutations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of the loop 's tertiary structure by Ser mutations of these Cys residues either prevented receptor assembly on the cell surface , or created receptors unable to be activated by agonists or to bind the competitive antagonist , strychnine .
	manualset3
248364	5	426465	16	NULL	NULL	0	NULL	Cys residues	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of the loop 's tertiary structure by Ser mutations of these Cys residues either prevented receptor assembly on the cell surface , or created receptors unable to be activated by agonists or to bind the competitive antagonist , strychnine .
	manualset3
248365	6	426465	16	NULL	NULL	0	NULL	receptor assembly	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of the loop 's tertiary structure by Ser mutations of these Cys residues either prevented receptor assembly on the cell surface , or created receptors unable to be activated by agonists or to bind the competitive antagonist , strychnine .
	manualset3
248368	7	426465	16	NULL	NULL	0	NULL	receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of the loop 's tertiary structure by Ser mutations of these Cys residues either prevented receptor assembly on the cell surface , or created receptors unable to be activated by agonists or to bind the competitive antagonist , strychnine .
	manualset3
248375	8	426465	16	NULL	NULL	0	NULL	agonists	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of the loop 's tertiary structure by Ser mutations of these Cys residues either prevented receptor assembly on the cell surface , or created receptors unable to be activated by agonists or to bind the competitive antagonist , strychnine .
	manualset3
248377	9	426465	16	NULL	NULL	0	NULL	bind	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of the loop 's tertiary structure by Ser mutations of these Cys residues either prevented receptor assembly on the cell surface , or created receptors unable to be activated by agonists or to bind the competitive antagonist , strychnine .
	manualset3
248379	10	426465	16	NULL	NULL	0	NULL	competitive antagonist	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of the loop 's tertiary structure by Ser mutations of these Cys residues either prevented receptor assembly on the cell surface , or created receptors unable to be activated by agonists or to bind the competitive antagonist , strychnine .
	manualset3
248380	11	426465	16	NULL	NULL	0	NULL	strychnine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of the loop 's tertiary structure by Ser mutations of these Cys residues either prevented receptor assembly on the cell surface , or created receptors unable to be activated by agonists or to bind the competitive antagonist , strychnine .
	manualset3
248381	1	426466	16	NULL	NULL	0	NULL	Disruption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of vanS by IS1216V in a clinical isolate of Enterococcus faecium with VanA glycopeptide resistance .
	manualset3
248382	2	426466	16	NULL	NULL	0	NULL	vanS	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of vanS by IS1216V in a clinical isolate of Enterococcus faecium with VanA glycopeptide resistance .
	manualset3
248383	3	426466	16	NULL	NULL	0	NULL	IS1216V	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of vanS by IS1216V in a clinical isolate of Enterococcus faecium with VanA glycopeptide resistance .
	manualset3
248414	4	426466	16	NULL	NULL	0	NULL	clinical isolate	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of vanS by IS1216V in a clinical isolate of Enterococcus faecium with VanA glycopeptide resistance .
	manualset3
248415	5	426466	16	NULL	NULL	0	NULL	Enterococcus faecium	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of vanS by IS1216V in a clinical isolate of Enterococcus faecium with VanA glycopeptide resistance .
	manualset3
248416	6	426466	16	NULL	NULL	0	NULL	VanA glycopeptide resistance	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Disruption of vanS by IS1216V in a clinical isolate of Enterococcus faecium with VanA glycopeptide resistance .
	manualset3
248417	1	426467	16	NULL	NULL	0	NULL	resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissecting resistance to endocrine therapy in breast cancer .
	manualset3
248418	2	426467	16	NULL	NULL	0	NULL	endocrine therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissecting resistance to endocrine therapy in breast cancer .
	manualset3
248420	3	426467	16	NULL	NULL	0	NULL	breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissecting resistance to endocrine therapy in breast cancer .
	manualset3
248428	1	426468	16	NULL	NULL	0	NULL	Dissection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissection of the inhibition of cardiac ryanodine receptors by human glutathione transferase GSTM2-2 .
	manualset3
248429	2	426468	16	NULL	NULL	0	NULL	inhibition	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissection of the inhibition of cardiac ryanodine receptors by human glutathione transferase GSTM2-2 .
	manualset3
248431	3	426468	16	NULL	NULL	0	NULL	cardiac ryanodine receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissection of the inhibition of cardiac ryanodine receptors by human glutathione transferase GSTM2-2 .
	manualset3
248433	4	426468	16	NULL	NULL	0	NULL	human glutathione transferase GSTM2-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissection of the inhibition of cardiac ryanodine receptors by human glutathione transferase GSTM2-2 .
	manualset3
248434	1	426469	16	NULL	NULL	0	NULL	Dissection	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissection of the underlying signaling mechanism revealed that rHP986 induces both TNFR1 and Fas expression to lead to apoptosis .
	manualset3
248435	2	426469	16	NULL	NULL	0	NULL	signaling mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissection of the underlying signaling mechanism revealed that rHP986 induces both TNFR1 and Fas expression to lead to apoptosis .
	manualset3
248436	3	426469	16	NULL	NULL	0	NULL	rHP986	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissection of the underlying signaling mechanism revealed that rHP986 induces both TNFR1 and Fas expression to lead to apoptosis .
	manualset3
248437	4	426469	16	NULL	NULL	0	NULL	TNFR1 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissection of the underlying signaling mechanism revealed that rHP986 induces both TNFR1 and Fas expression to lead to apoptosis .
	manualset3
248438	5	426469	16	NULL	NULL	0	NULL	Fas expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissection of the underlying signaling mechanism revealed that rHP986 induces both TNFR1 and Fas expression to lead to apoptosis .
	manualset3
248439	6	426469	16	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissection of the underlying signaling mechanism revealed that rHP986 induces both TNFR1 and Fas expression to lead to apoptosis .
	manualset3
248440	1	426470	16	NULL	NULL	0	NULL	information	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Disseminating information using an anesthesiology consultant report : impact on patient perceptions of quality of care .
	manualset3
248441	2	426470	16	NULL	NULL	0	NULL	anesthesiology consultant report 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Disseminating information using an anesthesiology consultant report : impact on patient perceptions of quality of care .
	manualset3
248442	3	426470	16	NULL	NULL	0	NULL	patient perceptions	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Disseminating information using an anesthesiology consultant report : impact on patient perceptions of quality of care .
	manualset3
248443	4	426470	16	NULL	NULL	0	NULL	quality	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Disseminating information using an anesthesiology consultant report : impact on patient perceptions of quality of care .
	manualset3
248444	5	426470	16	NULL	NULL	0	NULL	 care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Disseminating information using an anesthesiology consultant report : impact on patient perceptions of quality of care .
	manualset3
248445	1	426471	16	NULL	NULL	0	NULL	Dissipation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissipation of mitochondrial membrane potential , release of mitochondrial cytochrome c into cytosol , and subsequent induction of pro-caspase-9 and -3 processing preceded apoptosis in HL-60 cells , confirmed by DNA fragmentation , chromatin condensation , changes in the cell membrane and the appearance of a sub-G1 DNA peak .
	manualset3
248446	2	426471	16	NULL	NULL	0	NULL	mitochondrial membrane potential	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissipation of mitochondrial membrane potential , release of mitochondrial cytochrome c into cytosol , and subsequent induction of pro-caspase-9 and -3 processing preceded apoptosis in HL-60 cells , confirmed by DNA fragmentation , chromatin condensation , changes in the cell membrane and the appearance of a sub-G1 DNA peak .
	manualset3
248447	3	426471	16	NULL	NULL	0	NULL	release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissipation of mitochondrial membrane potential , release of mitochondrial cytochrome c into cytosol , and subsequent induction of pro-caspase-9 and -3 processing preceded apoptosis in HL-60 cells , confirmed by DNA fragmentation , chromatin condensation , changes in the cell membrane and the appearance of a sub-G1 DNA peak .
	manualset3
248448	4	426471	16	NULL	NULL	0	NULL	mitochondrial cytochrome c	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissipation of mitochondrial membrane potential , release of mitochondrial cytochrome c into cytosol , and subsequent induction of pro-caspase-9 and -3 processing preceded apoptosis in HL-60 cells , confirmed by DNA fragmentation , chromatin condensation , changes in the cell membrane and the appearance of a sub-G1 DNA peak .
	manualset3
248449	5	426471	16	NULL	NULL	0	NULL	cytosol	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissipation of mitochondrial membrane potential , release of mitochondrial cytochrome c into cytosol , and subsequent induction of pro-caspase-9 and -3 processing preceded apoptosis in HL-60 cells , confirmed by DNA fragmentation , chromatin condensation , changes in the cell membrane and the appearance of a sub-G1 DNA peak .
	manualset3
248450	6	426471	16	NULL	NULL	0	NULL	induction 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissipation of mitochondrial membrane potential , release of mitochondrial cytochrome c into cytosol , and subsequent induction of pro-caspase-9 and -3 processing preceded apoptosis in HL-60 cells , confirmed by DNA fragmentation , chromatin condensation , changes in the cell membrane and the appearance of a sub-G1 DNA peak .
	manualset3
248451	7	426471	16	NULL	NULL	0	NULL	 pro-caspase-9  processing	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissipation of mitochondrial membrane potential , release of mitochondrial cytochrome c into cytosol , and subsequent induction of pro-caspase-9 and -3 processing preceded apoptosis in HL-60 cells , confirmed by DNA fragmentation , chromatin condensation , changes in the cell membrane and the appearance of a sub-G1 DNA peak .
	manualset3
248452	8	426471	16	NULL	NULL	0	NULL	-3 processing	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissipation of mitochondrial membrane potential , release of mitochondrial cytochrome c into cytosol , and subsequent induction of pro-caspase-9 and -3 processing preceded apoptosis in HL-60 cells , confirmed by DNA fragmentation , chromatin condensation , changes in the cell membrane and the appearance of a sub-G1 DNA peak .
	manualset3
248453	9	426471	16	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissipation of mitochondrial membrane potential , release of mitochondrial cytochrome c into cytosol , and subsequent induction of pro-caspase-9 and -3 processing preceded apoptosis in HL-60 cells , confirmed by DNA fragmentation , chromatin condensation , changes in the cell membrane and the appearance of a sub-G1 DNA peak .
	manualset3
248454	10	426471	16	NULL	NULL	0	NULL	 HL-60 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissipation of mitochondrial membrane potential , release of mitochondrial cytochrome c into cytosol , and subsequent induction of pro-caspase-9 and -3 processing preceded apoptosis in HL-60 cells , confirmed by DNA fragmentation , chromatin condensation , changes in the cell membrane and the appearance of a sub-G1 DNA peak .
	manualset3
248455	11	426471	16	NULL	NULL	0	NULL	DNA fragmentation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissipation of mitochondrial membrane potential , release of mitochondrial cytochrome c into cytosol , and subsequent induction of pro-caspase-9 and -3 processing preceded apoptosis in HL-60 cells , confirmed by DNA fragmentation , chromatin condensation , changes in the cell membrane and the appearance of a sub-G1 DNA peak .
	manualset3
248456	12	426471	16	NULL	NULL	0	NULL	chromatin condensation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissipation of mitochondrial membrane potential , release of mitochondrial cytochrome c into cytosol , and subsequent induction of pro-caspase-9 and -3 processing preceded apoptosis in HL-60 cells , confirmed by DNA fragmentation , chromatin condensation , changes in the cell membrane and the appearance of a sub-G1 DNA peak .
	manualset3
248457	13	426471	16	NULL	NULL	0	NULL	changes	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissipation of mitochondrial membrane potential , release of mitochondrial cytochrome c into cytosol , and subsequent induction of pro-caspase-9 and -3 processing preceded apoptosis in HL-60 cells , confirmed by DNA fragmentation , chromatin condensation , changes in the cell membrane and the appearance of a sub-G1 DNA peak .
	manualset3
248458	14	426471	16	NULL	NULL	0	NULL	cell membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissipation of mitochondrial membrane potential , release of mitochondrial cytochrome c into cytosol , and subsequent induction of pro-caspase-9 and -3 processing preceded apoptosis in HL-60 cells , confirmed by DNA fragmentation , chromatin condensation , changes in the cell membrane and the appearance of a sub-G1 DNA peak .
	manualset3
248459	15	426471	16	NULL	NULL	0	NULL	appearance	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissipation of mitochondrial membrane potential , release of mitochondrial cytochrome c into cytosol , and subsequent induction of pro-caspase-9 and -3 processing preceded apoptosis in HL-60 cells , confirmed by DNA fragmentation , chromatin condensation , changes in the cell membrane and the appearance of a sub-G1 DNA peak .
	manualset3
248460	16	426471	16	NULL	NULL	0	NULL	sub-G1 DNA peak	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissipation of mitochondrial membrane potential , release of mitochondrial cytochrome c into cytosol , and subsequent induction of pro-caspase-9 and -3 processing preceded apoptosis in HL-60 cells , confirmed by DNA fragmentation , chromatin condensation , changes in the cell membrane and the appearance of a sub-G1 DNA peak .
	manualset3
248461	1	426472	16	NULL	NULL	0	NULL	rat hippocampal neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissociated rat hippocampal neurons were plated on polylysine-coated glass cover slips and grown in culture for 1-4 weeks .
	manualset3
248462	2	426472	16	NULL	NULL	NULL	NULL	polylysine-coated glass cover slips	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dissociated rat hippocampal neurons were plated on polylysine-coated glass cover slips and grown in culture for 1-4 weeks .
	manualset3
248463	3	426472	16	NULL	NULL	0	NULL	culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissociated rat hippocampal neurons were plated on polylysine-coated glass cover slips and grown in culture for 1-4 weeks .
	manualset3
248464	4	426472	16	NULL	NULL	0	NULL	1-4 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissociated rat hippocampal neurons were plated on polylysine-coated glass cover slips and grown in culture for 1-4 weeks .
	manualset3
248465	1	426473	16	NULL	NULL	0	NULL	Dissociation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissociation of POMC peptides after self-injury predicts responses to centrally acting opiate blockers .
	manualset3
248466	2	426473	16	NULL	NULL	0	NULL	POMC peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissociation of POMC peptides after self-injury predicts responses to centrally acting opiate blockers .
	manualset3
248467	3	426473	16	NULL	NULL	0	NULL	self-injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissociation of POMC peptides after self-injury predicts responses to centrally acting opiate blockers .
	manualset3
248468	4	426473	16	NULL	NULL	0	NULL	responses	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissociation of POMC peptides after self-injury predicts responses to centrally acting opiate blockers .
	manualset3
248469	5	426473	16	NULL	NULL	NULL	NULL	opiate blockers	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dissociation of POMC peptides after self-injury predicts responses to centrally acting opiate blockers .
	manualset3
248476	1	426474	16	NULL	NULL	0	NULL	Dissociation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissociation of nystatin and amphotericin analogs : characterisation of minor anti-fungal macrolides .
	manualset3
248698	2	426474	16	NULL	NULL	0	NULL	nystatin analogs	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissociation of nystatin and amphotericin analogs : characterisation of minor anti-fungal macrolides .
	manualset3
248700	3	426474	16	NULL	NULL	0	NULL	amphotericin analogs	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissociation of nystatin and amphotericin analogs : characterisation of minor anti-fungal macrolides .
	manualset3
248702	4	426474	16	NULL	NULL	0	NULL	characterisation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissociation of nystatin and amphotericin analogs : characterisation of minor anti-fungal macrolides .
	manualset3
248707	5	426474	16	NULL	NULL	0	NULL	anti-fungal macrolides	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissociation of nystatin and amphotericin analogs : characterisation of minor anti-fungal macrolides .
	manualset3
248712	1	426475	16	NULL	NULL	0	NULL	Dissolved oxygen	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissolved oxygen , number of tillers , and rice height were negatively associated with the abundance ofAn .
	manualset3
248714	2	426475	16	NULL	NULL	0	NULL	number of tillers	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissolved oxygen , number of tillers , and rice height were negatively associated with the abundance ofAn .
	manualset3
248715	3	426475	16	NULL	NULL	0	NULL	rice height	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissolved oxygen , number of tillers , and rice height were negatively associated with the abundance ofAn .
	manualset3
248722	4	426475	16	NULL	NULL	0	NULL	abundance	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissolved oxygen , number of tillers , and rice height were negatively associated with the abundance ofAn .
	manualset3
248725	5	426475	16	NULL	NULL	0	NULL	An .	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dissolved oxygen , number of tillers , and rice height were negatively associated with the abundance ofAn .
	manualset3
248750	1	426476	16	NULL	NULL	0	NULL	Distal esophageal sphincter pressure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Distal esophageal sphincter pressure and length of sphincter exposed to the positive pressure environment of the abdomen was measured by esophageal infusion manometry .
	manualset3
248752	2	426476	16	NULL	NULL	0	NULL	 length of sphincter	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Distal esophageal sphincter pressure and length of sphincter exposed to the positive pressure environment of the abdomen was measured by esophageal infusion manometry .
	manualset3
248756	3	426476	16	NULL	NULL	NULL	NULL	positive pressure environment	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Distal esophageal sphincter pressure and length of sphincter exposed to the positive pressure environment of the abdomen was measured by esophageal infusion manometry .
	manualset3
248768	4	426476	16	NULL	NULL	0	NULL	abdomen	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Distal esophageal sphincter pressure and length of sphincter exposed to the positive pressure environment of the abdomen was measured by esophageal infusion manometry .
	manualset3
248769	5	426476	16	NULL	NULL	0	NULL	esophageal infusion manometry	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Distal esophageal sphincter pressure and length of sphincter exposed to the positive pressure environment of the abdomen was measured by esophageal infusion manometry .
	manualset3
248770	1	426477	16	NULL	NULL	0	NULL	Distance telescopes	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Distance telescopes : a survey of user success .
	manualset3
248771	2	426477	16	NULL	NULL	0	NULL	survey	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Distance telescopes : a survey of user success .
	manualset3
248772	3	426477	16	NULL	NULL	0	NULL	user	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Distance telescopes : a survey of user success .
	manualset3
248773	4	426477	16	NULL	NULL	0	NULL	success	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Distance telescopes : a survey of user success .
	manualset3
248774	1	426478	16	NULL	NULL	0	NULL	domains	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinct domains of paracingulin are involved in its targeting to the actin cytoskeleton and regulation of apical junction assembly .
	manualset3
248775	2	426478	16	NULL	NULL	0	NULL	paracingulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinct domains of paracingulin are involved in its targeting to the actin cytoskeleton and regulation of apical junction assembly .
	manualset3
248776	3	426478	16	NULL	NULL	0	NULL	actin cytoskeleton	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinct domains of paracingulin are involved in its targeting to the actin cytoskeleton and regulation of apical junction assembly .
	manualset3
248777	4	426478	16	NULL	NULL	NULL	NULL	regulation of apical junction assembly	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Distinct domains of paracingulin are involved in its targeting to the actin cytoskeleton and regulation of apical junction assembly .
	manualset3
248779	1	426479	16	NULL	NULL	0	NULL	case	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( On a case of acrocephalosyndactylia and conjectured primary chronic polyarthritis ) .
	manualset3
248780	2	426479	16	NULL	NULL	0	NULL	acrocephalosyndactylia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( On a case of acrocephalosyndactylia and conjectured primary chronic polyarthritis ) .
	manualset3
248781	3	426479	16	NULL	NULL	0	NULL	primary chronic polyarthritis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( On a case of acrocephalosyndactylia and conjectured primary chronic polyarthritis ) .
	manualset3
248782	1	426480	16	NULL	NULL	0	NULL	Distinct patterns	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinct patterns of Fas cell surface expression during development of T - or B-lymphocyte lineages in normal , scid , and mutant mice lacking or overexpressing p53 , bcl-2 , or rag-2 genes .
	manualset3
248783	2	426480	16	NULL	NULL	0	NULL	Fas cell surface expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinct patterns of Fas cell surface expression during development of T - or B-lymphocyte lineages in normal , scid , and mutant mice lacking or overexpressing p53 , bcl-2 , or rag-2 genes .
	manualset3
248784	3	426480	16	NULL	NULL	NULL	NULL	 development of T-lymphocyte lineages	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Distinct patterns of Fas cell surface expression during development of T - or B-lymphocyte lineages in normal , scid , and mutant mice lacking or overexpressing p53 , bcl-2 , or rag-2 genes .
	manualset3
248785	4	426480	16	NULL	NULL	NULL	NULL	development of B-lymphocyte lineages	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Distinct patterns of Fas cell surface expression during development of T - or B-lymphocyte lineages in normal , scid , and mutant mice lacking or overexpressing p53 , bcl-2 , or rag-2 genes .
	manualset3
248786	5	426480	16	NULL	NULL	0	NULL	normal mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinct patterns of Fas cell surface expression during development of T - or B-lymphocyte lineages in normal , scid , and mutant mice lacking or overexpressing p53 , bcl-2 , or rag-2 genes .
	manualset3
248787	6	426480	16	NULL	NULL	0	NULL	scid mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinct patterns of Fas cell surface expression during development of T - or B-lymphocyte lineages in normal , scid , and mutant mice lacking or overexpressing p53 , bcl-2 , or rag-2 genes .
	manualset3
248788	7	426480	16	NULL	NULL	0	NULL	mutant mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinct patterns of Fas cell surface expression during development of T - or B-lymphocyte lineages in normal , scid , and mutant mice lacking or overexpressing p53 , bcl-2 , or rag-2 genes .
	manualset3
250927	8	426480	16	NULL	NULL	0	NULL	p53 genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinct patterns of Fas cell surface expression during development of T - or B-lymphocyte lineages in normal , scid , and mutant mice lacking or overexpressing p53 , bcl-2 , or rag-2 genes .
	manualset3
250928	9	426480	16	NULL	NULL	0	NULL	bcl-2 genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinct patterns of Fas cell surface expression during development of T - or B-lymphocyte lineages in normal , scid , and mutant mice lacking or overexpressing p53 , bcl-2 , or rag-2 genes .
	manualset3
250929	10	426480	16	NULL	NULL	0	NULL	rag-2 genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinct patterns of Fas cell surface expression during development of T - or B-lymphocyte lineages in normal , scid , and mutant mice lacking or overexpressing p53 , bcl-2 , or rag-2 genes .
	manualset3
248789	1	426481	16	NULL	NULL	0	NULL	viral sequence elements	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinct viral sequence elements mediate expression and derepression in phloem and activation in mesophyll , suggesting that TrAP interacts with different components of the cellular transcription machinery to accomplish CP gene expression in different cell types , and underscoring the intricacy and complexity of virus-host interactions .
	manualset3
248790	2	426481	16	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinct viral sequence elements mediate expression and derepression in phloem and activation in mesophyll , suggesting that TrAP interacts with different components of the cellular transcription machinery to accomplish CP gene expression in different cell types , and underscoring the intricacy and complexity of virus-host interactions .
	manualset3
248791	3	426481	16	NULL	NULL	0	NULL	derepression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinct viral sequence elements mediate expression and derepression in phloem and activation in mesophyll , suggesting that TrAP interacts with different components of the cellular transcription machinery to accomplish CP gene expression in different cell types , and underscoring the intricacy and complexity of virus-host interactions .
	manualset3
248792	4	426481	16	NULL	NULL	0	NULL	phloem	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinct viral sequence elements mediate expression and derepression in phloem and activation in mesophyll , suggesting that TrAP interacts with different components of the cellular transcription machinery to accomplish CP gene expression in different cell types , and underscoring the intricacy and complexity of virus-host interactions .
	manualset3
248793	5	426481	16	NULL	NULL	0	NULL	activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinct viral sequence elements mediate expression and derepression in phloem and activation in mesophyll , suggesting that TrAP interacts with different components of the cellular transcription machinery to accomplish CP gene expression in different cell types , and underscoring the intricacy and complexity of virus-host interactions .
	manualset3
248794	6	426481	16	NULL	NULL	0	NULL	mesophyll	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinct viral sequence elements mediate expression and derepression in phloem and activation in mesophyll , suggesting that TrAP interacts with different components of the cellular transcription machinery to accomplish CP gene expression in different cell types , and underscoring the intricacy and complexity of virus-host interactions .
	manualset3
248795	7	426481	16	NULL	NULL	0	NULL	TrAP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinct viral sequence elements mediate expression and derepression in phloem and activation in mesophyll , suggesting that TrAP interacts with different components of the cellular transcription machinery to accomplish CP gene expression in different cell types , and underscoring the intricacy and complexity of virus-host interactions .
	manualset3
248796	8	426481	16	NULL	NULL	0	NULL	components	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinct viral sequence elements mediate expression and derepression in phloem and activation in mesophyll , suggesting that TrAP interacts with different components of the cellular transcription machinery to accomplish CP gene expression in different cell types , and underscoring the intricacy and complexity of virus-host interactions .
	manualset3
248797	9	426481	16	NULL	NULL	0	NULL	cellular transcription machinery	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinct viral sequence elements mediate expression and derepression in phloem and activation in mesophyll , suggesting that TrAP interacts with different components of the cellular transcription machinery to accomplish CP gene expression in different cell types , and underscoring the intricacy and complexity of virus-host interactions .
	manualset3
248798	10	426481	16	NULL	NULL	0	NULL	CP gene expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinct viral sequence elements mediate expression and derepression in phloem and activation in mesophyll , suggesting that TrAP interacts with different components of the cellular transcription machinery to accomplish CP gene expression in different cell types , and underscoring the intricacy and complexity of virus-host interactions .
	manualset3
248799	11	426481	16	NULL	NULL	0	NULL	cell types	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinct viral sequence elements mediate expression and derepression in phloem and activation in mesophyll , suggesting that TrAP interacts with different components of the cellular transcription machinery to accomplish CP gene expression in different cell types , and underscoring the intricacy and complexity of virus-host interactions .
	manualset3
248800	12	426481	16	NULL	NULL	0	NULL	intricacy	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinct viral sequence elements mediate expression and derepression in phloem and activation in mesophyll , suggesting that TrAP interacts with different components of the cellular transcription machinery to accomplish CP gene expression in different cell types , and underscoring the intricacy and complexity of virus-host interactions .
	manualset3
248801	13	426481	16	NULL	NULL	0	NULL	complexity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinct viral sequence elements mediate expression and derepression in phloem and activation in mesophyll , suggesting that TrAP interacts with different components of the cellular transcription machinery to accomplish CP gene expression in different cell types , and underscoring the intricacy and complexity of virus-host interactions .
	manualset3
248802	14	426481	16	NULL	NULL	0	NULL	virus-host interactions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinct viral sequence elements mediate expression and derepression in phloem and activation in mesophyll , suggesting that TrAP interacts with different components of the cellular transcription machinery to accomplish CP gene expression in different cell types , and underscoring the intricacy and complexity of virus-host interactions .
	manualset3
248803	1	426482	16	NULL	NULL	0	NULL	Distinctive characteristics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinctive characteristics of non-small cell lung cancer ( NSCLC ) in the young : a surveillance , epidemiology , and end results ( SEER ) analysis .
	manualset3
248804	2	426482	16	NULL	NULL	0	NULL	non-small cell lung cancer ( NSCLC )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinctive characteristics of non-small cell lung cancer ( NSCLC ) in the young : a surveillance , epidemiology , and end results ( SEER ) analysis .
	manualset3
248805	3	426482	16	NULL	NULL	0	NULL	young	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinctive characteristics of non-small cell lung cancer ( NSCLC ) in the young : a surveillance , epidemiology , and end results ( SEER ) analysis .
	manualset3
248806	4	426482	16	NULL	NULL	0	NULL	surveillance , epidemiology , and end results ( SEER ) analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinctive characteristics of non-small cell lung cancer ( NSCLC ) in the young : a surveillance , epidemiology , and end results ( SEER ) analysis .
	manualset3
248807	1	426483	16	NULL	NULL	0	NULL	different band shapes	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinctively different band shapes have been observed for phen and bpy complexes .
	manualset3
248808	2	426483	16	NULL	NULL	0	NULL	phen complexes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinctively different band shapes have been observed for phen and bpy complexes .
	manualset3
248809	3	426483	16	NULL	NULL	0	NULL	bpy complexes	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinctively different band shapes have been observed for phen and bpy complexes .
	manualset3
248810	1	426484	16	NULL	NULL	0	NULL	developmental patterns	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinctly different developmental patterns were observed for cis-IPTase and HMG-CoA reductase activity , and when sterol biosynthesis was drastically inhibited by lovastatin , the rate of synthesis of Dol-P was slightly higher in the presence of the drug .
	manualset3
248811	2	426484	16	NULL	NULL	0	NULL	cis-IPTase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinctly different developmental patterns were observed for cis-IPTase and HMG-CoA reductase activity , and when sterol biosynthesis was drastically inhibited by lovastatin , the rate of synthesis of Dol-P was slightly higher in the presence of the drug .
	manualset3
248812	3	426484	16	NULL	NULL	0	NULL	HMG-CoA reductase activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinctly different developmental patterns were observed for cis-IPTase and HMG-CoA reductase activity , and when sterol biosynthesis was drastically inhibited by lovastatin , the rate of synthesis of Dol-P was slightly higher in the presence of the drug .
	manualset3
248813	4	426484	16	NULL	NULL	0	NULL	sterol biosynthesis	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinctly different developmental patterns were observed for cis-IPTase and HMG-CoA reductase activity , and when sterol biosynthesis was drastically inhibited by lovastatin , the rate of synthesis of Dol-P was slightly higher in the presence of the drug .
	manualset3
248814	5	426484	16	NULL	NULL	0	NULL	lovastatin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinctly different developmental patterns were observed for cis-IPTase and HMG-CoA reductase activity , and when sterol biosynthesis was drastically inhibited by lovastatin , the rate of synthesis of Dol-P was slightly higher in the presence of the drug .
	manualset3
248815	6	426484	16	NULL	NULL	0	NULL	rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinctly different developmental patterns were observed for cis-IPTase and HMG-CoA reductase activity , and when sterol biosynthesis was drastically inhibited by lovastatin , the rate of synthesis of Dol-P was slightly higher in the presence of the drug .
	manualset3
248816	7	426484	16	NULL	NULL	0	NULL	synthesis of Dol-P	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinctly different developmental patterns were observed for cis-IPTase and HMG-CoA reductase activity , and when sterol biosynthesis was drastically inhibited by lovastatin , the rate of synthesis of Dol-P was slightly higher in the presence of the drug .
	manualset3
248817	8	426484	16	NULL	NULL	0	NULL	presence	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinctly different developmental patterns were observed for cis-IPTase and HMG-CoA reductase activity , and when sterol biosynthesis was drastically inhibited by lovastatin , the rate of synthesis of Dol-P was slightly higher in the presence of the drug .
	manualset3
248818	9	426484	16	NULL	NULL	0	NULL	drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinctly different developmental patterns were observed for cis-IPTase and HMG-CoA reductase activity , and when sterol biosynthesis was drastically inhibited by lovastatin , the rate of synthesis of Dol-P was slightly higher in the presence of the drug .
	manualset3
248819	1	426485	16	NULL	NULL	0	NULL	Service Scroll presentation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinguished Service Scroll presentation to Henry C. Beebe by Frederick B. Lehman , AAO immediate past president .
	manualset3
248820	2	426485	16	NULL	NULL	0	NULL	Henry C. Beebe	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinguished Service Scroll presentation to Henry C. Beebe by Frederick B. Lehman , AAO immediate past president .
	manualset3
248821	3	426485	16	NULL	NULL	0	NULL	Frederick B. Lehman	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinguished Service Scroll presentation to Henry C. Beebe by Frederick B. Lehman , AAO immediate past president .
	manualset3
248822	4	426485	16	NULL	NULL	0	NULL	AAO	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinguished Service Scroll presentation to Henry C. Beebe by Frederick B. Lehman , AAO immediate past president .
	manualset3
248823	5	426485	16	NULL	NULL	0	NULL	president	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Distinguished Service Scroll presentation to Henry C. Beebe by Frederick B. Lehman , AAO immediate past president .
	manualset3
248834	1	426486	16	NULL	NULL	0	NULL	Distribution	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Distribution of florfenicol resistance genes fexA and cfr among chloramphenicol-resistant Staphylococcus isolates .
	manualset3
248835	2	426486	16	NULL	NULL	0	NULL	 florfenicol resistance 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Distribution of florfenicol resistance genes fexA and cfr among chloramphenicol-resistant Staphylococcus isolates .
	manualset3
248836	3	426486	16	NULL	NULL	0	NULL	genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Distribution of florfenicol resistance genes fexA and cfr among chloramphenicol-resistant Staphylococcus isolates .
	manualset3
248837	4	426486	16	NULL	NULL	0	NULL	 fexA	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Distribution of florfenicol resistance genes fexA and cfr among chloramphenicol-resistant Staphylococcus isolates .
	manualset3
248838	5	426486	16	NULL	NULL	0	NULL	cfr	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Distribution of florfenicol resistance genes fexA and cfr among chloramphenicol-resistant Staphylococcus isolates .
	manualset3
248839	6	426486	16	NULL	NULL	0	NULL	chloramphenicol-resistant Staphylococcus isolates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Distribution of florfenicol resistance genes fexA and cfr among chloramphenicol-resistant Staphylococcus isolates .
	manualset3
248840	1	426487	16	NULL	NULL	NULL	NULL	Distribution of positive cellsDistribution	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Distribution of positive cells in the epiblast was mosaic , whereas all cells of the forming hypoblast expressed the FGF-2 proteins .
	manualset3
248861	2	426487	16	NULL	NULL	0	NULL	epiblast	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Distribution of positive cells in the epiblast was mosaic , whereas all cells of the forming hypoblast expressed the FGF-2 proteins .
	manualset3
248863	3	426487	16	NULL	NULL	0	NULL	mosaic	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Distribution of positive cells in the epiblast was mosaic , whereas all cells of the forming hypoblast expressed the FGF-2 proteins .
	manualset3
248867	4	426487	16	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Distribution of positive cells in the epiblast was mosaic , whereas all cells of the forming hypoblast expressed the FGF-2 proteins .
	manualset3
248870	5	426487	16	NULL	NULL	0	NULL	hypoblast	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Distribution of positive cells in the epiblast was mosaic , whereas all cells of the forming hypoblast expressed the FGF-2 proteins .
	manualset3
248873	6	426487	16	NULL	NULL	0	NULL	FGF-2 proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Distribution of positive cells in the epiblast was mosaic , whereas all cells of the forming hypoblast expressed the FGF-2 proteins .
	manualset3
248881	1	426488	16	NULL	NULL	0	NULL	Distribution	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Distribution of respiratory mucin proteins in human nasal mucosa .
	manualset3
248884	2	426488	16	NULL	NULL	0	NULL	respiratory mucin proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Distribution of respiratory mucin proteins in human nasal mucosa .
	manualset3
248887	3	426488	16	NULL	NULL	0	NULL	human nasal mucosa	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Distribution of respiratory mucin proteins in human nasal mucosa .
	manualset3
248905	1	426489	16	NULL	NULL	0	NULL	Distribution	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Distribution of total progesterone receptor levels in various segments and tissues of the normal human uterus : the effect of short-term estrogen administration .
	manualset3
248912	2	426489	16	NULL	NULL	NULL	NULL	total progesterone receptor levels	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Distribution of total progesterone receptor levels in various segments and tissues of the normal human uterus : the effect of short-term estrogen administration .
	manualset3
248913	3	426489	16	NULL	NULL	0	NULL	segments	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Distribution of total progesterone receptor levels in various segments and tissues of the normal human uterus : the effect of short-term estrogen administration .
	manualset3
248914	4	426489	16	NULL	NULL	0	NULL	tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Distribution of total progesterone receptor levels in various segments and tissues of the normal human uterus : the effect of short-term estrogen administration .
	manualset3
248915	5	426489	16	NULL	NULL	0	NULL	human uterus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Distribution of total progesterone receptor levels in various segments and tissues of the normal human uterus : the effect of short-term estrogen administration .
	manualset3
248916	6	426489	16	NULL	NULL	0	NULL	effect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Distribution of total progesterone receptor levels in various segments and tissues of the normal human uterus : the effect of short-term estrogen administration .
	manualset3
248917	7	426489	16	NULL	NULL	0	NULL	short-term estrogen administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Distribution of total progesterone receptor levels in various segments and tissues of the normal human uterus : the effect of short-term estrogen administration .
	manualset3
248918	1	426490	16	NULL	NULL	0	NULL	Disturbances	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Disturbances in the operation of ion channels in these settings can alter normal physiology and cause disease .
	manualset3
248919	2	426490	16	NULL	NULL	0	NULL	operation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Disturbances in the operation of ion channels in these settings can alter normal physiology and cause disease .
	manualset3
248920	3	426490	16	NULL	NULL	0	NULL	ion channels	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Disturbances in the operation of ion channels in these settings can alter normal physiology and cause disease .
	manualset3
248921	4	426490	16	NULL	NULL	0	NULL	settings	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Disturbances in the operation of ion channels in these settings can alter normal physiology and cause disease .
	manualset3
248922	5	426490	16	NULL	NULL	0	NULL	normal physiology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Disturbances in the operation of ion channels in these settings can alter normal physiology and cause disease .
	manualset3
248923	6	426490	16	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Disturbances in the operation of ion channels in these settings can alter normal physiology and cause disease .
	manualset3
248924	1	426491	16	NULL	NULL	0	NULL	Disturbed chemical neurotransmission	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Disturbed chemical neurotransmission and sudden infant death syndrome -- the peripheral arterial chemoreceptors as an example .
	manualset3
248925	2	426491	16	NULL	NULL	0	NULL	sudden infant death syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Disturbed chemical neurotransmission and sudden infant death syndrome -- the peripheral arterial chemoreceptors as an example .
	manualset3
248926	3	426491	16	NULL	NULL	0	NULL	peripheral arterial chemoreceptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Disturbed chemical neurotransmission and sudden infant death syndrome -- the peripheral arterial chemoreceptors as an example .
	manualset3
248927	4	426491	16	NULL	NULL	0	NULL	example	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Disturbed chemical neurotransmission and sudden infant death syndrome -- the peripheral arterial chemoreceptors as an example .
	manualset3
248928	1	426492	16	NULL	NULL	0	NULL	Ditazole ( 4 , 5-diphenyl-2-bis - ( 2-hydroxyethyl ) - aminoxazol )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Ditazole ( 4 , 5-diphenyl-2-bis - ( 2-hydroxyethyl ) - aminoxazol ) is a new drug shown to inhibit prostaglandin release from rat platelets .
	manualset3
248929	2	426492	16	NULL	NULL	0	NULL	drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Ditazole ( 4 , 5-diphenyl-2-bis - ( 2-hydroxyethyl ) - aminoxazol ) is a new drug shown to inhibit prostaglandin release from rat platelets .
	manualset3
248930	3	426492	16	NULL	NULL	0	NULL	prostaglandin release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Ditazole ( 4 , 5-diphenyl-2-bis - ( 2-hydroxyethyl ) - aminoxazol ) is a new drug shown to inhibit prostaglandin release from rat platelets .
	manualset3
248931	4	426492	16	NULL	NULL	0	NULL	rat platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Ditazole ( 4 , 5-diphenyl-2-bis - ( 2-hydroxyethyl ) - aminoxazol ) is a new drug shown to inhibit prostaglandin release from rat platelets .
	manualset3
248932	1	426493	16	NULL	NULL	0	NULL	Diuresis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Diuresis and natriuresis following acute pneumothorax in very low birthweight infants .
	manualset3
248933	2	426493	16	NULL	NULL	0	NULL	natriuresis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Diuresis and natriuresis following acute pneumothorax in very low birthweight infants .
	manualset3
248934	3	426493	16	NULL	NULL	0	NULL	acute pneumothorax	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Diuresis and natriuresis following acute pneumothorax in very low birthweight infants .
	manualset3
248935	4	426493	16	NULL	NULL	0	NULL	low birthweight	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Diuresis and natriuresis following acute pneumothorax in very low birthweight infants .
	manualset3
248936	5	426493	16	NULL	NULL	0	NULL	infants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Diuresis and natriuresis following acute pneumothorax in very low birthweight infants .
	manualset3
248937	1	426494	16	NULL	NULL	0	NULL	DivIVA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	DivIVA is a conserved protein in Gram-positive bacteria and involved in various processes related to cell growth , cell division and spore formation .
	manualset3
248938	2	426494	16	NULL	NULL	0	NULL	conserved protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	DivIVA is a conserved protein in Gram-positive bacteria and involved in various processes related to cell growth , cell division and spore formation .
	manualset3
248939	3	426494	16	NULL	NULL	0	NULL	Gram-positive bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	DivIVA is a conserved protein in Gram-positive bacteria and involved in various processes related to cell growth , cell division and spore formation .
	manualset3
248940	4	426494	16	NULL	NULL	0	NULL	processes	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	DivIVA is a conserved protein in Gram-positive bacteria and involved in various processes related to cell growth , cell division and spore formation .
	manualset3
248941	5	426494	16	NULL	NULL	0	NULL	cell growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	DivIVA is a conserved protein in Gram-positive bacteria and involved in various processes related to cell growth , cell division and spore formation .
	manualset3
248942	6	426494	16	NULL	NULL	0	NULL	cell division	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	DivIVA is a conserved protein in Gram-positive bacteria and involved in various processes related to cell growth , cell division and spore formation .
	manualset3
248943	7	426494	16	NULL	NULL	0	NULL	spore formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	DivIVA is a conserved protein in Gram-positive bacteria and involved in various processes related to cell growth , cell division and spore formation .
	manualset3
248944	1	426495	16	NULL	NULL	0	NULL	Divalent cation ATPases	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Divalent cation ATPases were prepared from rat brain synaptic vesicles , synaptosomal plasma membranes , and plasma membranes from the brain stem and sciatic nerve and tested for optimal stimulation by Mn2 + , Mg2 + , or Ca2 + .
	manualset3
249095	2	426495	16	NULL	NULL	0	NULL	rat brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Divalent cation ATPases were prepared from rat brain synaptic vesicles , synaptosomal plasma membranes , and plasma membranes from the brain stem and sciatic nerve and tested for optimal stimulation by Mn2 + , Mg2 + , or Ca2 + .
	manualset3
249096	3	426495	16	NULL	NULL	0	NULL	synaptic vesicles	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Divalent cation ATPases were prepared from rat brain synaptic vesicles , synaptosomal plasma membranes , and plasma membranes from the brain stem and sciatic nerve and tested for optimal stimulation by Mn2 + , Mg2 + , or Ca2 + .
	manualset3
249097	4	426495	16	NULL	NULL	0	NULL	synaptosomal plasma membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Divalent cation ATPases were prepared from rat brain synaptic vesicles , synaptosomal plasma membranes , and plasma membranes from the brain stem and sciatic nerve and tested for optimal stimulation by Mn2 + , Mg2 + , or Ca2 + .
	manualset3
249098	5	426495	16	NULL	NULL	0	NULL	plasma membranes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Divalent cation ATPases were prepared from rat brain synaptic vesicles , synaptosomal plasma membranes , and plasma membranes from the brain stem and sciatic nerve and tested for optimal stimulation by Mn2 + , Mg2 + , or Ca2 + .
	manualset3
249099	6	426495	16	NULL	NULL	0	NULL	brain stem	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Divalent cation ATPases were prepared from rat brain synaptic vesicles , synaptosomal plasma membranes , and plasma membranes from the brain stem and sciatic nerve and tested for optimal stimulation by Mn2 + , Mg2 + , or Ca2 + .
	manualset3
249100	7	426495	16	NULL	NULL	0	NULL	sciatic nerve	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Divalent cation ATPases were prepared from rat brain synaptic vesicles , synaptosomal plasma membranes , and plasma membranes from the brain stem and sciatic nerve and tested for optimal stimulation by Mn2 + , Mg2 + , or Ca2 + .
	manualset3
249101	8	426495	16	NULL	NULL	0	NULL	optimal stimulation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Divalent cation ATPases were prepared from rat brain synaptic vesicles , synaptosomal plasma membranes , and plasma membranes from the brain stem and sciatic nerve and tested for optimal stimulation by Mn2 + , Mg2 + , or Ca2 + .
	manualset3
249102	9	426495	16	NULL	NULL	0	NULL	Mn2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Divalent cation ATPases were prepared from rat brain synaptic vesicles , synaptosomal plasma membranes , and plasma membranes from the brain stem and sciatic nerve and tested for optimal stimulation by Mn2 + , Mg2 + , or Ca2 + .
	manualset3
249103	10	426495	16	NULL	NULL	0	NULL	Mg2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Divalent cation ATPases were prepared from rat brain synaptic vesicles , synaptosomal plasma membranes , and plasma membranes from the brain stem and sciatic nerve and tested for optimal stimulation by Mn2 + , Mg2 + , or Ca2 + .
	manualset3
249104	11	426495	16	NULL	NULL	0	NULL	Ca2 + 	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Divalent cation ATPases were prepared from rat brain synaptic vesicles , synaptosomal plasma membranes , and plasma membranes from the brain stem and sciatic nerve and tested for optimal stimulation by Mn2 + , Mg2 + , or Ca2 + .
	manualset3
249105	1	426496	16	NULL	NULL	0	NULL	Divalent cations	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Divalent cations such as Cd2 + , Co2 + , and Mn2 + ( 0.1-3 .0 mM ) blocked this enhancement in a concentration-dependent manner .
	manualset3
249106	2	426496	16	NULL	NULL	0	NULL	Cd2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Divalent cations such as Cd2 + , Co2 + , and Mn2 + ( 0.1-3 .0 mM ) blocked this enhancement in a concentration-dependent manner .
	manualset3
249107	3	426496	16	NULL	NULL	0	NULL	Co2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Divalent cations such as Cd2 + , Co2 + , and Mn2 + ( 0.1-3 .0 mM ) blocked this enhancement in a concentration-dependent manner .
	manualset3
249108	4	426496	16	NULL	NULL	0	NULL	Mn2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	Divalent cations such as Cd2 + , Co2 + , and Mn2 + ( 0.1-3 .0 mM ) blocked this enhancement in a concentration-dependent manner .
	manualset3
249109	5	426496	16	NULL	NULL	0	NULL	0.1-3 .0 mM	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Divalent cations such as Cd2 + , Co2 + , and Mn2 + ( 0.1-3 .0 mM ) blocked this enhancement in a concentration-dependent manner .
	manualset3
249110	6	426496	16	NULL	NULL	0	NULL	enhancement	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Divalent cations such as Cd2 + , Co2 + , and Mn2 + ( 0.1-3 .0 mM ) blocked this enhancement in a concentration-dependent manner .
	manualset3
249111	7	426496	16	NULL	NULL	0	NULL	concentration-dependent manner	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Divalent cations such as Cd2 + , Co2 + , and Mn2 + ( 0.1-3 .0 mM ) blocked this enhancement in a concentration-dependent manner .
	manualset3
249112	1	426497	16	NULL	NULL	0	NULL	Divergence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Divergence of the mitochondrial leucyl tRNA synthetase genes in two closely related yeasts Saccharomyces cerevisiae and Saccharomyces douglasii : a paradigm of incipient evolution .
	manualset3
249113	2	426497	16	NULL	NULL	0	NULL	mitochondrial leucyl tRNA synthetase genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Divergence of the mitochondrial leucyl tRNA synthetase genes in two closely related yeasts Saccharomyces cerevisiae and Saccharomyces douglasii : a paradigm of incipient evolution .
	manualset3
249114	3	426497	16	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Divergence of the mitochondrial leucyl tRNA synthetase genes in two closely related yeasts Saccharomyces cerevisiae and Saccharomyces douglasii : a paradigm of incipient evolution .
	manualset3
249115	4	426497	16	NULL	NULL	0	NULL	yeasts	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Divergence of the mitochondrial leucyl tRNA synthetase genes in two closely related yeasts Saccharomyces cerevisiae and Saccharomyces douglasii : a paradigm of incipient evolution .
	manualset3
249116	5	426497	16	NULL	NULL	0	NULL	Saccharomyces cerevisiae	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Divergence of the mitochondrial leucyl tRNA synthetase genes in two closely related yeasts Saccharomyces cerevisiae and Saccharomyces douglasii : a paradigm of incipient evolution .
	manualset3
249117	6	426497	16	NULL	NULL	0	NULL	Saccharomyces douglasii	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Divergence of the mitochondrial leucyl tRNA synthetase genes in two closely related yeasts Saccharomyces cerevisiae and Saccharomyces douglasii : a paradigm of incipient evolution .
	manualset3
249118	7	426497	16	NULL	NULL	0	NULL	paradigm	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Divergence of the mitochondrial leucyl tRNA synthetase genes in two closely related yeasts Saccharomyces cerevisiae and Saccharomyces douglasii : a paradigm of incipient evolution .
	manualset3
249119	8	426497	16	NULL	NULL	0	NULL	incipient evolution	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Divergence of the mitochondrial leucyl tRNA synthetase genes in two closely related yeasts Saccharomyces cerevisiae and Saccharomyces douglasii : a paradigm of incipient evolution .
	manualset3
249120	1	426498	16	NULL	NULL	0	NULL	species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Diverse species of pathogenic Gram-negative bacteria use secretion systems to export a variety of protein toxins and virulence factors that help establish and maintain infection .
	manualset3
249121	2	426498	16	NULL	NULL	0	NULL	Gram-negative bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Diverse species of pathogenic Gram-negative bacteria use secretion systems to export a variety of protein toxins and virulence factors that help establish and maintain infection .
	manualset3
249122	3	426498	16	NULL	NULL	NULL	NULL	secretion systems	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Diverse species of pathogenic Gram-negative bacteria use secretion systems to export a variety of protein toxins and virulence factors that help establish and maintain infection .
	manualset3
249123	4	426498	16	NULL	NULL	0	NULL	variety	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Diverse species of pathogenic Gram-negative bacteria use secretion systems to export a variety of protein toxins and virulence factors that help establish and maintain infection .
	manualset3
249124	5	426498	16	NULL	NULL	0	NULL	protein toxins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Diverse species of pathogenic Gram-negative bacteria use secretion systems to export a variety of protein toxins and virulence factors that help establish and maintain infection .
	manualset3
249125	6	426498	16	NULL	NULL	0	NULL	virulence factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Diverse species of pathogenic Gram-negative bacteria use secretion systems to export a variety of protein toxins and virulence factors that help establish and maintain infection .
	manualset3
249126	7	426498	16	NULL	NULL	0	NULL	infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Diverse species of pathogenic Gram-negative bacteria use secretion systems to export a variety of protein toxins and virulence factors that help establish and maintain infection .
	manualset3
249127	1	426499	16	NULL	NULL	0	NULL	Diversity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Diversity and challenges in the management of maternity care for migrant women .
	manualset3
249128	2	426499	16	NULL	NULL	0	NULL	challenges	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Diversity and challenges in the management of maternity care for migrant women .
	manualset3
249129	3	426499	16	NULL	NULL	0	NULL	management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Diversity and challenges in the management of maternity care for migrant women .
	manualset3
249130	4	426499	16	NULL	NULL	0	NULL	maternity care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Diversity and challenges in the management of maternity care for migrant women .
	manualset3
249131	5	426499	16	NULL	NULL	0	NULL	migrant women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Diversity and challenges in the management of maternity care for migrant women .
	manualset3
249132	1	426500	16	NULL	NULL	0	NULL	Diverticulum	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Diverticulum of the urethra in the female .
	manualset3
249133	2	426500	16	NULL	NULL	0	NULL	urethra	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Diverticulum of the urethra in the female .
	manualset3
249134	3	426500	16	NULL	NULL	0	NULL	female	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Diverticulum of the urethra in the female .
	manualset3
249135	1	426501	16	NULL	NULL	0	NULL	attention	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dividing attention during prospective memory retrieval substantially reduced prospective memory performance ( Experiment 3 ) .
	manualset3
249136	2	426501	16	NULL	NULL	0	NULL	prospective memory retrieval	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dividing attention during prospective memory retrieval substantially reduced prospective memory performance ( Experiment 3 ) .
	manualset3
249137	3	426501	16	NULL	NULL	0	NULL	reduced prospective memory performance	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Dividing attention during prospective memory retrieval substantially reduced prospective memory performance ( Experiment 3 ) .
	manualset3
249138	4	426501	16	NULL	NULL	0	NULL	Experiment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dividing attention during prospective memory retrieval substantially reduced prospective memory performance ( Experiment 3 ) .
	manualset3
249139	5	426501	16	NULL	NULL	0	NULL	3	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dividing attention during prospective memory retrieval substantially reduced prospective memory performance ( Experiment 3 ) .
	manualset3
249140	1	426502	16	NULL	NULL	0	NULL	DmFoxF	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	DmFoxF , a novel Drosophila fork head factor expressed in visceral mesoderm .
	manualset3
249141	2	426502	16	NULL	NULL	0	NULL	Drosophila fork head factor	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	DmFoxF , a novel Drosophila fork head factor expressed in visceral mesoderm .
	manualset3
249142	3	426502	16	NULL	NULL	0	NULL	visceral mesoderm	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	DmFoxF , a novel Drosophila fork head factor expressed in visceral mesoderm .
	manualset3
249143	1	426503	16	NULL	NULL	0	NULL	DmsA	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	DmsA belongs to the Type II subclass of Mo-bisPGD-containing catalytic subunits that is distinguished from the Type I subclass by having three rather than two residues between the first two Cys residues coordinating FS0 and a conserved Arg residue rather than a Lys residue following the fourth cluster coordinating Cys .
	manualset3
249144	2	426503	16	NULL	NULL	0	NULL	Type II subclass	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	DmsA belongs to the Type II subclass of Mo-bisPGD-containing catalytic subunits that is distinguished from the Type I subclass by having three rather than two residues between the first two Cys residues coordinating FS0 and a conserved Arg residue rather than a Lys residue following the fourth cluster coordinating Cys .
	manualset3
249145	3	426503	16	NULL	NULL	0	NULL	Mo-bisPGD-containing catalytic subunits	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	DmsA belongs to the Type II subclass of Mo-bisPGD-containing catalytic subunits that is distinguished from the Type I subclass by having three rather than two residues between the first two Cys residues coordinating FS0 and a conserved Arg residue rather than a Lys residue following the fourth cluster coordinating Cys .
	manualset3
249146	4	426503	16	NULL	NULL	0	NULL	Type I subclass	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	DmsA belongs to the Type II subclass of Mo-bisPGD-containing catalytic subunits that is distinguished from the Type I subclass by having three rather than two residues between the first two Cys residues coordinating FS0 and a conserved Arg residue rather than a Lys residue following the fourth cluster coordinating Cys .
	manualset3
249147	5	426503	16	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	DmsA belongs to the Type II subclass of Mo-bisPGD-containing catalytic subunits that is distinguished from the Type I subclass by having three rather than two residues between the first two Cys residues coordinating FS0 and a conserved Arg residue rather than a Lys residue following the fourth cluster coordinating Cys .
	manualset3
249148	6	426503	16	NULL	NULL	0	NULL	two residues	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	DmsA belongs to the Type II subclass of Mo-bisPGD-containing catalytic subunits that is distinguished from the Type I subclass by having three rather than two residues between the first two Cys residues coordinating FS0 and a conserved Arg residue rather than a Lys residue following the fourth cluster coordinating Cys .
	manualset3
249149	7	426503	16	NULL	NULL	0	NULL	two Cys residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	DmsA belongs to the Type II subclass of Mo-bisPGD-containing catalytic subunits that is distinguished from the Type I subclass by having three rather than two residues between the first two Cys residues coordinating FS0 and a conserved Arg residue rather than a Lys residue following the fourth cluster coordinating Cys .
	manualset3
249150	8	426503	16	NULL	NULL	0	NULL	coordinating FS0	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	DmsA belongs to the Type II subclass of Mo-bisPGD-containing catalytic subunits that is distinguished from the Type I subclass by having three rather than two residues between the first two Cys residues coordinating FS0 and a conserved Arg residue rather than a Lys residue following the fourth cluster coordinating Cys .
	manualset3
249151	9	426503	16	NULL	NULL	0	NULL	Arg residue	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	DmsA belongs to the Type II subclass of Mo-bisPGD-containing catalytic subunits that is distinguished from the Type I subclass by having three rather than two residues between the first two Cys residues coordinating FS0 and a conserved Arg residue rather than a Lys residue following the fourth cluster coordinating Cys .
	manualset3
249152	10	426503	16	NULL	NULL	0	NULL	Lys residue	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	DmsA belongs to the Type II subclass of Mo-bisPGD-containing catalytic subunits that is distinguished from the Type I subclass by having three rather than two residues between the first two Cys residues coordinating FS0 and a conserved Arg residue rather than a Lys residue following the fourth cluster coordinating Cys .
	manualset3
249153	11	426503	16	NULL	NULL	0	NULL	fourth cluster	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	DmsA belongs to the Type II subclass of Mo-bisPGD-containing catalytic subunits that is distinguished from the Type I subclass by having three rather than two residues between the first two Cys residues coordinating FS0 and a conserved Arg residue rather than a Lys residue following the fourth cluster coordinating Cys .
	manualset3
249154	12	426503	16	NULL	NULL	0	NULL	Cys	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	DmsA belongs to the Type II subclass of Mo-bisPGD-containing catalytic subunits that is distinguished from the Type I subclass by having three rather than two residues between the first two Cys residues coordinating FS0 and a conserved Arg residue rather than a Lys residue following the fourth cluster coordinating Cys .
	manualset3
249155	1	426504	16	NULL	NULL	0	NULL	electron microscopic findings	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( On electron microscopic findings in diabetic angiopathy ) .
	manualset3
249156	2	426504	16	NULL	NULL	0	NULL	diabetic angiopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( On electron microscopic findings in diabetic angiopathy ) .
	manualset3
249157	1	426505	16	NULL	NULL	0	NULL	legume storage proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Do legume storage proteins play a role in defending seeds against bruchids ?
	manualset3
249158	2	426505	16	NULL	NULL	NULL	NULL	role	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Do legume storage proteins play a role in defending seeds against bruchids ?
	manualset3
249159	3	426505	16	NULL	NULL	0	NULL	seeds	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Do legume storage proteins play a role in defending seeds against bruchids ?
	manualset3
249160	4	426505	16	NULL	NULL	0	NULL	bruchids	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Do legume storage proteins play a role in defending seeds against bruchids ?
	manualset3
249161	1	426506	16	NULL	NULL	0	NULL	risk factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Do risk factors for schizophrenia predispose to emigration ?
	manualset3
249162	2	426506	16	NULL	NULL	0	NULL	schizophrenia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Do risk factors for schizophrenia predispose to emigration ?
	manualset3
249163	3	426506	16	NULL	NULL	0	NULL	emigration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Do risk factors for schizophrenia predispose to emigration ?
	manualset3
249164	1	426507	16	NULL	NULL	0	NULL	MDL-1 cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Do MDL-1 cells play a broad role in acute inflammation ?
	manualset3
249165	2	426507	16	NULL	NULL	NULL	NULL	role	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Do MDL-1 cells play a broad role in acute inflammation ?
	manualset3
249166	3	426507	16	NULL	NULL	0	NULL	acute inflammation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Do MDL-1 cells play a broad role in acute inflammation ?
	manualset3
249167	1	426508	16	NULL	NULL	0	NULL	people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Do people with acquired brain impairment benefit from additional therapy specifically directed at the hand ?
	manualset3
249168	2	426508	16	NULL	NULL	0	NULL	acquired brain impairment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Do people with acquired brain impairment benefit from additional therapy specifically directed at the hand ?
	manualset3
249169	3	426508	16	NULL	NULL	NULL	NULL	benefit	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Do people with acquired brain impairment benefit from additional therapy specifically directed at the hand ?
	manualset3
249170	4	426508	16	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Do people with acquired brain impairment benefit from additional therapy specifically directed at the hand ?
	manualset3
249171	5	426508	16	NULL	NULL	0	NULL	hand	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Do people with acquired brain impairment benefit from additional therapy specifically directed at the hand ?
	manualset3
249172	1	426509	16	NULL	NULL	0	NULL	spices	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Do spices increase acceptability of therapeutic diets .
	manualset3
249173	2	426509	16	NULL	NULL	0	NULL	acceptability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Do spices increase acceptability of therapeutic diets .
	manualset3
249174	3	426509	16	NULL	NULL	0	NULL	therapeutic diets	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Do spices increase acceptability of therapeutic diets .
	manualset3
249175	1	426510	16	NULL	NULL	0	NULL	computed tomography scans	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Do routinely repeated computed tomography scans in traumatic brain injury influence management ?
	manualset3
249176	2	426510	16	NULL	NULL	0	NULL	traumatic brain injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Do routinely repeated computed tomography scans in traumatic brain injury influence management ?
	manualset3
249177	3	426510	16	NULL	NULL	0	NULL	management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Do routinely repeated computed tomography scans in traumatic brain injury influence management ?
	manualset3
249178	1	426511	16	NULL	NULL	NULL	NULL	postmortem decomposition	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( On postmortem decomposition of organic sulfur compounds in relation to redox potential ; the formation of mercaptans and thioethers ) .
	manualset3
249179	2	426511	16	NULL	NULL	0	NULL	organic sulfur compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( On postmortem decomposition of organic sulfur compounds in relation to redox potential ; the formation of mercaptans and thioethers ) .
	manualset3
249180	3	426511	16	NULL	NULL	0	NULL	relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	( On postmortem decomposition of organic sulfur compounds in relation to redox potential ; the formation of mercaptans and thioethers ) .
	manualset3
249181	4	426511	16	NULL	NULL	0	NULL	redox potential	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( On postmortem decomposition of organic sulfur compounds in relation to redox potential ; the formation of mercaptans and thioethers ) .
	manualset3
249182	5	426511	16	NULL	NULL	0	NULL	formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( On postmortem decomposition of organic sulfur compounds in relation to redox potential ; the formation of mercaptans and thioethers ) .
	manualset3
249183	6	426511	16	NULL	NULL	0	NULL	mercaptans	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( On postmortem decomposition of organic sulfur compounds in relation to redox potential ; the formation of mercaptans and thioethers ) .
	manualset3
249184	7	426511	16	NULL	NULL	0	NULL	thioethers	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( On postmortem decomposition of organic sulfur compounds in relation to redox potential ; the formation of mercaptans and thioethers ) .
	manualset3
249185	1	426512	16	NULL	NULL	0	NULL	Dobutamine echocardiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Dobutamine echocardiography has been found to be more specific than thallium scintigraphy for predicting functional recovery after revascularization .
	manualset3
249186	2	426512	16	NULL	NULL	0	NULL	specific	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Dobutamine echocardiography has been found to be more specific than thallium scintigraphy for predicting functional recovery after revascularization .
	manualset3
249187	3	426512	16	NULL	NULL	0	NULL	thallium scintigraphy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Dobutamine echocardiography has been found to be more specific than thallium scintigraphy for predicting functional recovery after revascularization .
	manualset3
249188	4	426512	16	NULL	NULL	0	NULL	functional recovery	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dobutamine echocardiography has been found to be more specific than thallium scintigraphy for predicting functional recovery after revascularization .
	manualset3
249189	5	426512	16	NULL	NULL	0	NULL	revascularization	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Dobutamine echocardiography has been found to be more specific than thallium scintigraphy for predicting functional recovery after revascularization .
	manualset3
249347	1	426513	16	NULL	NULL	0	NULL	Docosahexaenoic acid ( DHA )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Docosahexaenoic acid ( DHA ) was shown to be involved in the regulation of expression of drug metabolizing enzymes ( DMEs ) in rat primary hepatocytes in response to xenobiotics .
	manualset3
249348	2	426513	16	NULL	NULL	0	NULL	regulation of expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Docosahexaenoic acid ( DHA ) was shown to be involved in the regulation of expression of drug metabolizing enzymes ( DMEs ) in rat primary hepatocytes in response to xenobiotics .
	manualset3
249349	3	426513	16	NULL	NULL	0	NULL	drug metabolizing enzymes ( DMEs )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Docosahexaenoic acid ( DHA ) was shown to be involved in the regulation of expression of drug metabolizing enzymes ( DMEs ) in rat primary hepatocytes in response to xenobiotics .
	manualset3
249352	4	426513	16	NULL	NULL	0	NULL	rat primary hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Docosahexaenoic acid ( DHA ) was shown to be involved in the regulation of expression of drug metabolizing enzymes ( DMEs ) in rat primary hepatocytes in response to xenobiotics .
	manualset3
249356	5	426513	16	NULL	NULL	NULL	NULL	response to xenobiotics	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Docosahexaenoic acid ( DHA ) was shown to be involved in the regulation of expression of drug metabolizing enzymes ( DMEs ) in rat primary hepatocytes in response to xenobiotics .
	manualset3
249246	1	426514	16	NULL	NULL	0	NULL	Docosahexaenoic acid release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Docosahexaenoic acid release proceeds simultaneously with arachidonic acid ( 20 : 4 n-6 ) release and prostaglandin liberation from astrocytes .
	manualset3
249249	2	426514	16	NULL	NULL	0	NULL	arachidonic acid ( 20 : 4 n-6 ) release	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Docosahexaenoic acid release proceeds simultaneously with arachidonic acid ( 20 : 4 n-6 ) release and prostaglandin liberation from astrocytes .
	manualset3
249250	3	426514	16	NULL	NULL	0	NULL	prostaglandin liberation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Docosahexaenoic acid release proceeds simultaneously with arachidonic acid ( 20 : 4 n-6 ) release and prostaglandin liberation from astrocytes .
	manualset3
249254	4	426514	16	NULL	NULL	0	NULL	astrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Docosahexaenoic acid release proceeds simultaneously with arachidonic acid ( 20 : 4 n-6 ) release and prostaglandin liberation from astrocytes .
	manualset3
249260	1	426515	16	NULL	NULL	0	NULL	asbestos	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Does asbestos cause laryngeal cancer ?
	manualset3
249262	2	426515	16	NULL	NULL	0	NULL	laryngeal cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Does asbestos cause laryngeal cancer ?
	manualset3
249273	1	426516	16	NULL	NULL	0	NULL	aprotinin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Does aprotinin preserve platelets in children with acyanogenic congenital heart disease undergone surgery with cardiopulmonary bypass ?
	manualset3
249274	2	426516	16	NULL	NULL	0	NULL	preserve	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Does aprotinin preserve platelets in children with acyanogenic congenital heart disease undergone surgery with cardiopulmonary bypass ?
	manualset3
249275	3	426516	16	NULL	NULL	0	NULL	platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Does aprotinin preserve platelets in children with acyanogenic congenital heart disease undergone surgery with cardiopulmonary bypass ?
	manualset3
249276	4	426516	16	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Does aprotinin preserve platelets in children with acyanogenic congenital heart disease undergone surgery with cardiopulmonary bypass ?
	manualset3
249277	5	426516	16	NULL	NULL	0	NULL	acyanogenic congenital heart disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Does aprotinin preserve platelets in children with acyanogenic congenital heart disease undergone surgery with cardiopulmonary bypass ?
	manualset3
249278	6	426516	16	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Does aprotinin preserve platelets in children with acyanogenic congenital heart disease undergone surgery with cardiopulmonary bypass ?
	manualset3
249279	7	426516	16	NULL	NULL	0	NULL	cardiopulmonary bypass	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Does aprotinin preserve platelets in children with acyanogenic congenital heart disease undergone surgery with cardiopulmonary bypass ?
	manualset3
249280	1	426517	16	NULL	NULL	0	NULL	body height reduction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Does body height reduction influence interpretation of lung function in COPD patients ?
	manualset3
249281	2	426517	16	NULL	NULL	0	NULL	interpretation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Does body height reduction influence interpretation of lung function in COPD patients ?
	manualset3
249282	3	426517	16	NULL	NULL	0	NULL	lung function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Does body height reduction influence interpretation of lung function in COPD patients ?
	manualset3
249283	4	426517	16	NULL	NULL	NULL	NULL	COPD patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Does body height reduction influence interpretation of lung function in COPD patients ?
	manualset3
249284	1	426518	16	NULL	NULL	0	NULL	continuity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Does continuity of care matter ?
	manualset3
249285	2	426518	16	NULL	NULL	0	NULL	care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Does continuity of care matter ?
	manualset3
249286	1	426519	16	NULL	NULL	0	NULL	disturbance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Does disturbance and restoration of alpine grassland soils affect the genetic structure and diversity of bacterial and N2-fixing populations ?
	manualset3
249287	2	426519	16	NULL	NULL	0	NULL	restoration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Does disturbance and restoration of alpine grassland soils affect the genetic structure and diversity of bacterial and N2-fixing populations ?
	manualset3
249288	3	426519	16	NULL	NULL	0	NULL	genetic structure	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Does disturbance and restoration of alpine grassland soils affect the genetic structure and diversity of bacterial and N2-fixing populations ?
	manualset3
249289	4	426519	16	NULL	NULL	0	NULL	diversity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Does disturbance and restoration of alpine grassland soils affect the genetic structure and diversity of bacterial and N2-fixing populations ?
	manualset3
249290	5	426519	16	NULL	NULL	0	NULL	bacterial populations	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Does disturbance and restoration of alpine grassland soils affect the genetic structure and diversity of bacterial and N2-fixing populations ?
	manualset3
249291	6	426519	16	NULL	NULL	0	NULL	N2-fixing populations	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Does disturbance and restoration of alpine grassland soils affect the genetic structure and diversity of bacterial and N2-fixing populations ?
	manualset3
249372	1	426520	16	NULL	NULL	0	NULL	pressor regulation of blood circulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( On pressor and depressor regulation of blood circulation in resuscitation of the organism after clinical death ) .
	manualset3
249379	2	426520	16	NULL	NULL	0	NULL	depressor regulation of blood circulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( On pressor and depressor regulation of blood circulation in resuscitation of the organism after clinical death ) .
	manualset3
249382	3	426520	16	NULL	NULL	0	NULL	resuscitation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( On pressor and depressor regulation of blood circulation in resuscitation of the organism after clinical death ) .
	manualset3
249384	4	426520	16	NULL	NULL	0	NULL	organism	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( On pressor and depressor regulation of blood circulation in resuscitation of the organism after clinical death ) .
	manualset3
249387	5	426520	16	NULL	NULL	0	NULL	clinical death	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( On pressor and depressor regulation of blood circulation in resuscitation of the organism after clinical death ) .
	manualset3
249397	1	426521	16	NULL	NULL	0	NULL	dystonia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Does dystonia always include co-contraction ?
	manualset3
249402	2	426521	16	NULL	NULL	0	NULL	co-contraction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Does dystonia always include co-contraction ?
	manualset3
249408	1	426522	16	NULL	NULL	0	NULL	pre-exposure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Does pre-exposure of Aspergillus fumigatus to voriconazole or posaconazole in vitro affect its virulence and the in vivo activity of subsequent posaconazole or voriconazole , respectively ?
	manualset3
249411	2	426522	16	NULL	NULL	0	NULL	Aspergillus fumigatus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Does pre-exposure of Aspergillus fumigatus to voriconazole or posaconazole in vitro affect its virulence and the in vivo activity of subsequent posaconazole or voriconazole , respectively ?
	manualset3
249416	3	426522	16	NULL	NULL	0	NULL	voriconazole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Does pre-exposure of Aspergillus fumigatus to voriconazole or posaconazole in vitro affect its virulence and the in vivo activity of subsequent posaconazole or voriconazole , respectively ?
	manualset3
249418	4	426522	16	NULL	NULL	0	NULL	posaconazole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Does pre-exposure of Aspergillus fumigatus to voriconazole or posaconazole in vitro affect its virulence and the in vivo activity of subsequent posaconazole or voriconazole , respectively ?
	manualset3
249454	5	426522	16	NULL	NULL	0	NULL	virulence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Does pre-exposure of Aspergillus fumigatus to voriconazole or posaconazole in vitro affect its virulence and the in vivo activity of subsequent posaconazole or voriconazole , respectively ?
	manualset3
249455	6	426522	16	NULL	NULL	0	NULL	in vivo activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Does pre-exposure of Aspergillus fumigatus to voriconazole or posaconazole in vitro affect its virulence and the in vivo activity of subsequent posaconazole or voriconazole , respectively ?
	manualset3
249456	7	426522	16	NULL	NULL	0	NULL	posaconazole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Does pre-exposure of Aspergillus fumigatus to voriconazole or posaconazole in vitro affect its virulence and the in vivo activity of subsequent posaconazole or voriconazole , respectively ?
	manualset3
249457	8	426522	16	NULL	NULL	0	NULL	voriconazole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Does pre-exposure of Aspergillus fumigatus to voriconazole or posaconazole in vitro affect its virulence and the in vivo activity of subsequent posaconazole or voriconazole , respectively ?
	manualset3
249458	1	426523	16	NULL	NULL	0	NULL	prehospital care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Does prehospital care by physicians result in a better outcome than resuscitation by other EMS personnel ?
	manualset3
249459	2	426523	16	NULL	NULL	0	NULL	physicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Does prehospital care by physicians result in a better outcome than resuscitation by other EMS personnel ?
	manualset3
249460	3	426523	16	NULL	NULL	0	NULL	outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Does prehospital care by physicians result in a better outcome than resuscitation by other EMS personnel ?
	manualset3
249461	4	426523	16	NULL	NULL	0	NULL	resuscitation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Does prehospital care by physicians result in a better outcome than resuscitation by other EMS personnel ?
	manualset3
249462	5	426523	16	NULL	NULL	0	NULL	EMS personnel	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Does prehospital care by physicians result in a better outcome than resuscitation by other EMS personnel ?
	manualset3
249464	1	426524	16	NULL	NULL	0	NULL	history of violence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Does a history of violence influence treatment , self-help , and 1-year outcomes in substance use disorder patients ?
	manualset3
249465	2	426524	16	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Does a history of violence influence treatment , self-help , and 1-year outcomes in substance use disorder patients ?
	manualset3
249466	3	426524	16	NULL	NULL	0	NULL	self-help	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Does a history of violence influence treatment , self-help , and 1-year outcomes in substance use disorder patients ?
	manualset3
249467	4	426524	16	NULL	NULL	0	NULL	1-year	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Does a history of violence influence treatment , self-help , and 1-year outcomes in substance use disorder patients ?
	manualset3
249468	5	426524	16	NULL	NULL	0	NULL	outcomes	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Does a history of violence influence treatment , self-help , and 1-year outcomes in substance use disorder patients ?
	manualset3
249469	6	426524	16	NULL	NULL	0	NULL	substance use disorder patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Does a history of violence influence treatment , self-help , and 1-year outcomes in substance use disorder patients ?
	manualset3
249470	1	426525	16	NULL	NULL	0	NULL	gastroesophageal reflux	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Does gastroesophageal reflux contribute to the development of chronic sinusitis ?
	manualset3
249471	2	426525	16	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Does gastroesophageal reflux contribute to the development of chronic sinusitis ?
	manualset3
249472	3	426525	16	NULL	NULL	0	NULL	chronic sinusitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Does gastroesophageal reflux contribute to the development of chronic sinusitis ?
	manualset3
249473	1	426526	16	NULL	NULL	0	NULL	neoadjuvant hormonal therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Does neoadjuvant hormonal therapy improve urinary function when given to men with large prostates undergoing prostate brachytherapy ?
	manualset3
249474	2	426526	16	NULL	NULL	0	NULL	urinary function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Does neoadjuvant hormonal therapy improve urinary function when given to men with large prostates undergoing prostate brachytherapy ?
	manualset3
249475	3	426526	16	NULL	NULL	0	NULL	men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Does neoadjuvant hormonal therapy improve urinary function when given to men with large prostates undergoing prostate brachytherapy ?
	manualset3
249476	4	426526	16	NULL	NULL	0	NULL	large prostates	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Does neoadjuvant hormonal therapy improve urinary function when given to men with large prostates undergoing prostate brachytherapy ?
	manualset3
249477	5	426526	16	NULL	NULL	0	NULL	prostate brachytherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Does neoadjuvant hormonal therapy improve urinary function when given to men with large prostates undergoing prostate brachytherapy ?
	manualset3
249478	1	426527	16	NULL	NULL	NULL	NULL	Dog kidney proximal tubule cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dog and rat kidney proximal tubule cells in culture : responses to parathyroid hormone .
	manualset3
249479	2	426527	16	NULL	NULL	0	NULL	rat kidney proximal tubule cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Dog and rat kidney proximal tubule cells in culture : responses to parathyroid hormone .
	manualset3
249480	3	426527	16	NULL	NULL	0	NULL	culture	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Dog and rat kidney proximal tubule cells in culture : responses to parathyroid hormone .
	manualset3
249481	4	426527	16	NULL	NULL	0	NULL	responses to parathyroid hormone	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dog and rat kidney proximal tubule cells in culture : responses to parathyroid hormone .
	manualset3
249482	1	426528	16	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( On surgery of Dupuytren 's contracture ) .
	manualset3
249483	2	426528	16	NULL	NULL	0	NULL	Dupuytren 's contracture	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( On surgery of Dupuytren 's contracture ) .
	manualset3
249484	1	426529	16	NULL	NULL	0	NULL	Dogs	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Dogs showed no evidence of pain or distress at any point .
	manualset3
249485	2	426529	16	NULL	NULL	NULL	NULL	evidence of pain	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dogs showed no evidence of pain or distress at any point .
	manualset3
249487	4	426529	16	NULL	NULL	0	NULL	distress	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dogs showed no evidence of pain or distress at any point .
	manualset3
249488	5	426529	16	NULL	NULL	0	NULL	point	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Dogs showed no evidence of pain or distress at any point .
	manualset3
249489	1	426530	16	NULL	NULL	0	NULL	Domain 5 ( D5 )	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Domain 5 ( D5 ) is a highly conserved , largely helical substructure of group II introns that is essential for self-splicing .
	manualset3
249490	2	426530	16	NULL	NULL	0	NULL	helical substructure	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Domain 5 ( D5 ) is a highly conserved , largely helical substructure of group II introns that is essential for self-splicing .
	manualset3
249491	3	426530	16	NULL	NULL	0	NULL	group II introns	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Domain 5 ( D5 ) is a highly conserved , largely helical substructure of group II introns that is essential for self-splicing .
	manualset3
249492	4	426530	16	NULL	NULL	0	NULL	self-splicing	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Domain 5 ( D5 ) is a highly conserved , largely helical substructure of group II introns that is essential for self-splicing .
	manualset3
249493	1	426531	16	NULL	NULL	0	NULL	Domestic violence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Domestic violence , deportation , and women 's resistance : notes on managing inter-sectionality .
	manualset3
249494	2	426531	16	NULL	NULL	0	NULL	deportation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Domestic violence , deportation , and women 's resistance : notes on managing inter-sectionality .
	manualset3
249495	3	426531	16	NULL	NULL	0	NULL	women 's resistance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Domestic violence , deportation , and women 's resistance : notes on managing inter-sectionality .
	manualset3
249496	4	426531	16	NULL	NULL	NULL	NULL	notes	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Domestic violence , deportation , and women 's resistance : notes on managing inter-sectionality .
	manualset3
249497	5	426531	16	NULL	NULL	0	NULL	inter-sectionality	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Domestic violence , deportation , and women 's resistance : notes on managing inter-sectionality .
	manualset3
249498	1	426532	16	NULL	NULL	0	NULL	Dominant species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Dominant species in larval collections included Culex pipiens , Cx .
	manualset3
249499	2	426532	16	NULL	NULL	0	NULL	larval collections	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Dominant species in larval collections included Culex pipiens , Cx .
	manualset3
249500	3	426532	16	NULL	NULL	0	NULL	Culex pipiens	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Dominant species in larval collections included Culex pipiens , Cx .
	manualset3
249501	4	426532	16	NULL	NULL	0	NULL	Cx	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Dominant species in larval collections included Culex pipiens , Cx .
	manualset3
249502	1	426533	16	NULL	NULL	0	NULL	Dominantly-inherited adult-onset leukodystrophy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Dominantly-inherited adult-onset leukodystrophy with palatal tremor caused by a mutation in the glial fibrillary acidic protein gene .
	manualset3
249503	2	426533	16	NULL	NULL	0	NULL	palatal tremor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dominantly-inherited adult-onset leukodystrophy with palatal tremor caused by a mutation in the glial fibrillary acidic protein gene .
	manualset3
249504	3	426533	16	NULL	NULL	0	NULL	mutation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dominantly-inherited adult-onset leukodystrophy with palatal tremor caused by a mutation in the glial fibrillary acidic protein gene .
	manualset3
249505	4	426533	16	NULL	NULL	0	NULL	 glial fibrillary acidic protein gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Dominantly-inherited adult-onset leukodystrophy with palatal tremor caused by a mutation in the glial fibrillary acidic protein gene .
	manualset3
249506	1	426534	16	NULL	NULL	0	NULL	Domperidone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Domperidone ( n = 6 ) did not affect plasma ( K + ) at any time , but after propranolol ( n = 6 ) it increased by a mean ( S.E.M. ) of 0.39 ( 0.09 ) mmol l-1 ( P = 0.01 ) in normoxia and by a further 0.62 ( 0.28 ) mmol l-1 ( P = 0.08 ) at 60 min of hypoxia .
	manualset3
249507	2	426534	16	NULL	NULL	0	NULL	n = 6	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Domperidone ( n = 6 ) did not affect plasma ( K + ) at any time , but after propranolol ( n = 6 ) it increased by a mean ( S.E.M. ) of 0.39 ( 0.09 ) mmol l-1 ( P = 0.01 ) in normoxia and by a further 0.62 ( 0.28 ) mmol l-1 ( P = 0.08 ) at 60 min of hypoxia .
	manualset3
249508	3	426534	16	NULL	NULL	0	NULL	plasma ( K + )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Domperidone ( n = 6 ) did not affect plasma ( K + ) at any time , but after propranolol ( n = 6 ) it increased by a mean ( S.E.M. ) of 0.39 ( 0.09 ) mmol l-1 ( P = 0.01 ) in normoxia and by a further 0.62 ( 0.28 ) mmol l-1 ( P = 0.08 ) at 60 min of hypoxia .
	manualset3
249509	4	426534	16	NULL	NULL	0	NULL	time	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Domperidone ( n = 6 ) did not affect plasma ( K + ) at any time , but after propranolol ( n = 6 ) it increased by a mean ( S.E.M. ) of 0.39 ( 0.09 ) mmol l-1 ( P = 0.01 ) in normoxia and by a further 0.62 ( 0.28 ) mmol l-1 ( P = 0.08 ) at 60 min of hypoxia .
	manualset3
249510	5	426534	16	NULL	NULL	0	NULL	propranolol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Domperidone ( n = 6 ) did not affect plasma ( K + ) at any time , but after propranolol ( n = 6 ) it increased by a mean ( S.E.M. ) of 0.39 ( 0.09 ) mmol l-1 ( P = 0.01 ) in normoxia and by a further 0.62 ( 0.28 ) mmol l-1 ( P = 0.08 ) at 60 min of hypoxia .
	manualset3
249511	6	426534	16	NULL	NULL	0	NULL	n = 6	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Domperidone ( n = 6 ) did not affect plasma ( K + ) at any time , but after propranolol ( n = 6 ) it increased by a mean ( S.E.M. ) of 0.39 ( 0.09 ) mmol l-1 ( P = 0.01 ) in normoxia and by a further 0.62 ( 0.28 ) mmol l-1 ( P = 0.08 ) at 60 min of hypoxia .
	manualset3
249512	7	426534	16	NULL	NULL	0	NULL	mean ( S.E.M. )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Domperidone ( n = 6 ) did not affect plasma ( K + ) at any time , but after propranolol ( n = 6 ) it increased by a mean ( S.E.M. ) of 0.39 ( 0.09 ) mmol l-1 ( P = 0.01 ) in normoxia and by a further 0.62 ( 0.28 ) mmol l-1 ( P = 0.08 ) at 60 min of hypoxia .
	manualset3
249513	8	426534	16	NULL	NULL	0	NULL	0.39 ( 0.09 ) mmol l-1 ( P = 0.01 )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Domperidone ( n = 6 ) did not affect plasma ( K + ) at any time , but after propranolol ( n = 6 ) it increased by a mean ( S.E.M. ) of 0.39 ( 0.09 ) mmol l-1 ( P = 0.01 ) in normoxia and by a further 0.62 ( 0.28 ) mmol l-1 ( P = 0.08 ) at 60 min of hypoxia .
	manualset3
249514	9	426534	16	NULL	NULL	0	NULL	normoxia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Domperidone ( n = 6 ) did not affect plasma ( K + ) at any time , but after propranolol ( n = 6 ) it increased by a mean ( S.E.M. ) of 0.39 ( 0.09 ) mmol l-1 ( P = 0.01 ) in normoxia and by a further 0.62 ( 0.28 ) mmol l-1 ( P = 0.08 ) at 60 min of hypoxia .
	manualset3
249515	10	426534	16	NULL	NULL	0	NULL	0.62 ( 0.28 ) mmol l-1 ( P = 0.08 )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Domperidone ( n = 6 ) did not affect plasma ( K + ) at any time , but after propranolol ( n = 6 ) it increased by a mean ( S.E.M. ) of 0.39 ( 0.09 ) mmol l-1 ( P = 0.01 ) in normoxia and by a further 0.62 ( 0.28 ) mmol l-1 ( P = 0.08 ) at 60 min of hypoxia .
	manualset3
249516	11	426534	16	NULL	NULL	0	NULL	60 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Domperidone ( n = 6 ) did not affect plasma ( K + ) at any time , but after propranolol ( n = 6 ) it increased by a mean ( S.E.M. ) of 0.39 ( 0.09 ) mmol l-1 ( P = 0.01 ) in normoxia and by a further 0.62 ( 0.28 ) mmol l-1 ( P = 0.08 ) at 60 min of hypoxia .
	manualset3
249517	12	426534	16	NULL	NULL	0	NULL	hypoxia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Domperidone ( n = 6 ) did not affect plasma ( K + ) at any time , but after propranolol ( n = 6 ) it increased by a mean ( S.E.M. ) of 0.39 ( 0.09 ) mmol l-1 ( P = 0.01 ) in normoxia and by a further 0.62 ( 0.28 ) mmol l-1 ( P = 0.08 ) at 60 min of hypoxia .
	manualset3
249518	1	426535	16	NULL	NULL	0	NULL	action	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the action of propranolol ( inderal ) on the contractile function of the heart ) .
	manualset3
249519	2	426535	16	NULL	NULL	0	NULL	propranolol ( inderal )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the action of propranolol ( inderal ) on the contractile function of the heart ) .
	manualset3
249520	3	426535	16	NULL	NULL	0	NULL	contractile function	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the action of propranolol ( inderal ) on the contractile function of the heart ) .
	manualset3
249521	4	426535	16	NULL	NULL	0	NULL	heart	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the action of propranolol ( inderal ) on the contractile function of the heart ) .
	manualset3
249522	1	426536	16	NULL	NULL	0	NULL	Donor age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Donor age , parity , and donor sex match were not associated with transplantation outcome .
	manualset3
249523	2	426536	16	NULL	NULL	0	NULL	Donor parity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Donor age , parity , and donor sex match were not associated with transplantation outcome .
	manualset3
249524	3	426536	16	NULL	NULL	0	NULL	donor sex match	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Donor age , parity , and donor sex match were not associated with transplantation outcome .
	manualset3
249525	4	426536	16	NULL	NULL	0	NULL	transplantation outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Donor age , parity , and donor sex match were not associated with transplantation outcome .
	manualset3
249559	1	426537	16	NULL	NULL	0	NULL	Dopamine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Dopamine ( 100 microg kg ( -1 ) min ( -1 ) intra-carotid , i.c. ) potentiated thrombin ( 90 u kg ( -1 ) , i.c. ) induced platelet accumulation in the cerebral vasculature whereas higher doses ( 1-2 mg kg ( -1 ) min ( -1 ) ) inhibited accumulation .
	manualset3
249562	2	426537	16	NULL	NULL	0	NULL	100 microg kg ( -1 ) min ( -1 )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Dopamine ( 100 microg kg ( -1 ) min ( -1 ) intra-carotid , i.c. ) potentiated thrombin ( 90 u kg ( -1 ) , i.c. ) induced platelet accumulation in the cerebral vasculature whereas higher doses ( 1-2 mg kg ( -1 ) min ( -1 ) ) inhibited accumulation .
	manualset3
249579	3	426537	16	NULL	NULL	0	NULL	potentiated thrombin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Dopamine ( 100 microg kg ( -1 ) min ( -1 ) intra-carotid , i.c. ) potentiated thrombin ( 90 u kg ( -1 ) , i.c. ) induced platelet accumulation in the cerebral vasculature whereas higher doses ( 1-2 mg kg ( -1 ) min ( -1 ) ) inhibited accumulation .
	manualset3
249580	4	426537	16	NULL	NULL	0	NULL	90 u kg ( -1 )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Dopamine ( 100 microg kg ( -1 ) min ( -1 ) intra-carotid , i.c. ) potentiated thrombin ( 90 u kg ( -1 ) , i.c. ) induced platelet accumulation in the cerebral vasculature whereas higher doses ( 1-2 mg kg ( -1 ) min ( -1 ) ) inhibited accumulation .
	manualset3
249581	5	426537	16	NULL	NULL	0	NULL	induced platelet accumulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dopamine ( 100 microg kg ( -1 ) min ( -1 ) intra-carotid , i.c. ) potentiated thrombin ( 90 u kg ( -1 ) , i.c. ) induced platelet accumulation in the cerebral vasculature whereas higher doses ( 1-2 mg kg ( -1 ) min ( -1 ) ) inhibited accumulation .
	manualset3
249583	6	426537	16	NULL	NULL	0	NULL	cerebral vasculature	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Dopamine ( 100 microg kg ( -1 ) min ( -1 ) intra-carotid , i.c. ) potentiated thrombin ( 90 u kg ( -1 ) , i.c. ) induced platelet accumulation in the cerebral vasculature whereas higher doses ( 1-2 mg kg ( -1 ) min ( -1 ) ) inhibited accumulation .
	manualset3
249586	7	426537	16	NULL	NULL	0	NULL	higher doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dopamine ( 100 microg kg ( -1 ) min ( -1 ) intra-carotid , i.c. ) potentiated thrombin ( 90 u kg ( -1 ) , i.c. ) induced platelet accumulation in the cerebral vasculature whereas higher doses ( 1-2 mg kg ( -1 ) min ( -1 ) ) inhibited accumulation .
	manualset3
249589	8	426537	16	NULL	NULL	0	NULL	1-2 mg kg ( -1 ) min ( -1 )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Dopamine ( 100 microg kg ( -1 ) min ( -1 ) intra-carotid , i.c. ) potentiated thrombin ( 90 u kg ( -1 ) , i.c. ) induced platelet accumulation in the cerebral vasculature whereas higher doses ( 1-2 mg kg ( -1 ) min ( -1 ) ) inhibited accumulation .
	manualset3
249590	9	426537	16	NULL	NULL	0	NULL	inhibited accumulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dopamine ( 100 microg kg ( -1 ) min ( -1 ) intra-carotid , i.c. ) potentiated thrombin ( 90 u kg ( -1 ) , i.c. ) induced platelet accumulation in the cerebral vasculature whereas higher doses ( 1-2 mg kg ( -1 ) min ( -1 ) ) inhibited accumulation .
	manualset3
249591	1	426538	16	NULL	NULL	0	NULL	Dopamine D1 receptor-mediated NMDA receptor insertion	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dopamine D1 receptor-mediated NMDA receptor insertion depends on Fyn but not Src kinase pathway in prefrontal cortical neurons .
	manualset3
249592	2	426538	16	NULL	NULL	0	NULL	Fyn kinase pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dopamine D1 receptor-mediated NMDA receptor insertion depends on Fyn but not Src kinase pathway in prefrontal cortical neurons .
	manualset3
249593	3	426538	16	NULL	NULL	0	NULL	Src kinase pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dopamine D1 receptor-mediated NMDA receptor insertion depends on Fyn but not Src kinase pathway in prefrontal cortical neurons .
	manualset3
249594	4	426538	16	NULL	NULL	0	NULL	prefrontal cortical neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Dopamine D1 receptor-mediated NMDA receptor insertion depends on Fyn but not Src kinase pathway in prefrontal cortical neurons .
	manualset3
249595	1	426539	16	NULL	NULL	0	NULL	Dopamine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Dopamine acts at the same receptors as noradrenaline in the rat isolated vas deferens .
	manualset3
249596	2	426539	16	NULL	NULL	0	NULL	receptors	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Dopamine acts at the same receptors as noradrenaline in the rat isolated vas deferens .
	manualset3
249597	3	426539	16	NULL	NULL	0	NULL	noradrenaline	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Dopamine acts at the same receptors as noradrenaline in the rat isolated vas deferens .
	manualset3
249598	4	426539	16	NULL	NULL	0	NULL	rat	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Dopamine acts at the same receptors as noradrenaline in the rat isolated vas deferens .
	manualset3
249599	5	426539	16	NULL	NULL	0	NULL	vas deferens	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Dopamine acts at the same receptors as noradrenaline in the rat isolated vas deferens .
	manualset3
249600	1	426540	16	NULL	NULL	0	NULL	Dopamine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Dopamine did not affect the increases in R ( L ) or the falls in C ( dyn ) produced by histamine .
	manualset3
249601	2	426540	16	NULL	NULL	NULL	NULL	increases in R ( L )	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dopamine did not affect the increases in R ( L ) or the falls in C ( dyn ) produced by histamine .
	manualset3
249602	3	426540	16	NULL	NULL	NULL	NULL	falls in C ( dyn )	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dopamine did not affect the increases in R ( L ) or the falls in C ( dyn ) produced by histamine .
	manualset3
249603	4	426540	16	NULL	NULL	NULL	NULL	histamine	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dopamine did not affect the increases in R ( L ) or the falls in C ( dyn ) produced by histamine .
	manualset3
249604	1	426541	16	NULL	NULL	0	NULL	Dopamine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Dopamine inhibited the induction of NAT activity by forskolin and IBMX , but not that elicited by 8-bromocyclic AMP .
	manualset3
249605	2	426541	16	NULL	NULL	0	NULL	induction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dopamine inhibited the induction of NAT activity by forskolin and IBMX , but not that elicited by 8-bromocyclic AMP .
	manualset3
249606	3	426541	16	NULL	NULL	0	NULL	NAT activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dopamine inhibited the induction of NAT activity by forskolin and IBMX , but not that elicited by 8-bromocyclic AMP .
	manualset3
249607	4	426541	16	NULL	NULL	0	NULL	forskolin	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Dopamine inhibited the induction of NAT activity by forskolin and IBMX , but not that elicited by 8-bromocyclic AMP .
	manualset3
249608	5	426541	16	NULL	NULL	0	NULL	IBMX	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Dopamine inhibited the induction of NAT activity by forskolin and IBMX , but not that elicited by 8-bromocyclic AMP .
	manualset3
249609	6	426541	16	NULL	NULL	0	NULL	 8-bromocyclic AMP	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Dopamine inhibited the induction of NAT activity by forskolin and IBMX , but not that elicited by 8-bromocyclic AMP .
	manualset3
249610	1	426542	16	NULL	NULL	0	NULL	Doppler-guided hemorrhoidal artery ligation with recto anal repair	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler-guided hemorrhoidal artery ligation with recto anal repair : a new technique for the treatment of symptomatic hemorrhoids .
	manualset3
249611	2	426542	16	NULL	NULL	NULL	NULL	technique	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Doppler-guided hemorrhoidal artery ligation with recto anal repair : a new technique for the treatment of symptomatic hemorrhoids .
	manualset3
249612	3	426542	16	NULL	NULL	0	NULL	 treatment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler-guided hemorrhoidal artery ligation with recto anal repair : a new technique for the treatment of symptomatic hemorrhoids .
	manualset3
249613	4	426542	16	NULL	NULL	0	NULL	symptomatic hemorrhoids	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler-guided hemorrhoidal artery ligation with recto anal repair : a new technique for the treatment of symptomatic hemorrhoids .
	manualset3
249614	1	426543	16	NULL	NULL	0	NULL	Doppler evaluation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler evaluation of changing cardiac dynamics during Cheyne-Stokes respiration .
	manualset3
249615	2	426543	16	NULL	NULL	0	NULL	cardiac dynamics	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler evaluation of changing cardiac dynamics during Cheyne-Stokes respiration .
	manualset3
249616	3	426543	16	NULL	NULL	0	NULL	Cheyne-Stokes respiration	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler evaluation of changing cardiac dynamics during Cheyne-Stokes respiration .
	manualset3
249617	1	426544	16	NULL	NULL	0	NULL	Doppler echocardiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler echocardiography would appear to be the best method of following up cardiac rhabdomyomas , and enabled the demonstration of partial regression of the largest tumor in one of these two cases .
	manualset3
249618	2	426544	16	NULL	NULL	0	NULL	method	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler echocardiography would appear to be the best method of following up cardiac rhabdomyomas , and enabled the demonstration of partial regression of the largest tumor in one of these two cases .
	manualset3
249619	3	426544	16	NULL	NULL	0	NULL	following up	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler echocardiography would appear to be the best method of following up cardiac rhabdomyomas , and enabled the demonstration of partial regression of the largest tumor in one of these two cases .
	manualset3
249620	4	426544	16	NULL	NULL	0	NULL	cardiac rhabdomyomas	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler echocardiography would appear to be the best method of following up cardiac rhabdomyomas , and enabled the demonstration of partial regression of the largest tumor in one of these two cases .
	manualset3
249621	5	426544	16	NULL	NULL	0	NULL	demonstration	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler echocardiography would appear to be the best method of following up cardiac rhabdomyomas , and enabled the demonstration of partial regression of the largest tumor in one of these two cases .
	manualset3
249622	6	426544	16	NULL	NULL	0	NULL	partial regression	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler echocardiography would appear to be the best method of following up cardiac rhabdomyomas , and enabled the demonstration of partial regression of the largest tumor in one of these two cases .
	manualset3
249623	7	426544	16	NULL	NULL	0	NULL	tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler echocardiography would appear to be the best method of following up cardiac rhabdomyomas , and enabled the demonstration of partial regression of the largest tumor in one of these two cases .
	manualset3
249624	8	426544	16	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler echocardiography would appear to be the best method of following up cardiac rhabdomyomas , and enabled the demonstration of partial regression of the largest tumor in one of these two cases .
	manualset3
249625	9	426544	16	NULL	NULL	0	NULL	two cases	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler echocardiography would appear to be the best method of following up cardiac rhabdomyomas , and enabled the demonstration of partial regression of the largest tumor in one of these two cases .
	manualset3
249626	1	426545	16	NULL	NULL	0	NULL	Doppler evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler evidence of persistent left atrial mechanical standstill with normal P-waves by electrocardiogram after biatrial CryoMaze procedure for atrial fibrillation .
	manualset3
249627	2	426545	16	NULL	NULL	0	NULL	persistent left atrial mechanical standstill	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler evidence of persistent left atrial mechanical standstill with normal P-waves by electrocardiogram after biatrial CryoMaze procedure for atrial fibrillation .
	manualset3
249628	3	426545	16	NULL	NULL	0	NULL	P-waves	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler evidence of persistent left atrial mechanical standstill with normal P-waves by electrocardiogram after biatrial CryoMaze procedure for atrial fibrillation .
	manualset3
249629	4	426545	16	NULL	NULL	0	NULL	electrocardiogram	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler evidence of persistent left atrial mechanical standstill with normal P-waves by electrocardiogram after biatrial CryoMaze procedure for atrial fibrillation .
	manualset3
249630	5	426545	16	NULL	NULL	0	NULL	biatrial CryoMaze procedure	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler evidence of persistent left atrial mechanical standstill with normal P-waves by electrocardiogram after biatrial CryoMaze procedure for atrial fibrillation .
	manualset3
249631	6	426545	16	NULL	NULL	0	NULL	atrial fibrillation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler evidence of persistent left atrial mechanical standstill with normal P-waves by electrocardiogram after biatrial CryoMaze procedure for atrial fibrillation .
	manualset3
249632	1	426546	16	NULL	NULL	0	NULL	Doppler sonography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler sonography and immunofluorescence studies showed that intramuscular implantation of isolated fraction of autologous bone marrow mononuclear cells in combination with laser tunneling of the muscles is most effective and can be recommended as a method of angiogenesis stimulation in non-reconstructable distal vascular pathology of the extremities .
	manualset3
249633	2	426546	16	NULL	NULL	0	NULL	immunofluorescence studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler sonography and immunofluorescence studies showed that intramuscular implantation of isolated fraction of autologous bone marrow mononuclear cells in combination with laser tunneling of the muscles is most effective and can be recommended as a method of angiogenesis stimulation in non-reconstructable distal vascular pathology of the extremities .
	manualset3
249634	3	426546	16	NULL	NULL	0	NULL	intramuscular implantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler sonography and immunofluorescence studies showed that intramuscular implantation of isolated fraction of autologous bone marrow mononuclear cells in combination with laser tunneling of the muscles is most effective and can be recommended as a method of angiogenesis stimulation in non-reconstructable distal vascular pathology of the extremities .
	manualset3
249635	4	426546	16	NULL	NULL	0	NULL	fraction	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler sonography and immunofluorescence studies showed that intramuscular implantation of isolated fraction of autologous bone marrow mononuclear cells in combination with laser tunneling of the muscles is most effective and can be recommended as a method of angiogenesis stimulation in non-reconstructable distal vascular pathology of the extremities .
	manualset3
249636	5	426546	16	NULL	NULL	0	NULL	autologous bone marrow mononuclear cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler sonography and immunofluorescence studies showed that intramuscular implantation of isolated fraction of autologous bone marrow mononuclear cells in combination with laser tunneling of the muscles is most effective and can be recommended as a method of angiogenesis stimulation in non-reconstructable distal vascular pathology of the extremities .
	manualset3
249637	6	426546	16	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler sonography and immunofluorescence studies showed that intramuscular implantation of isolated fraction of autologous bone marrow mononuclear cells in combination with laser tunneling of the muscles is most effective and can be recommended as a method of angiogenesis stimulation in non-reconstructable distal vascular pathology of the extremities .
	manualset3
249638	7	426546	16	NULL	NULL	0	NULL	laser tunneling	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler sonography and immunofluorescence studies showed that intramuscular implantation of isolated fraction of autologous bone marrow mononuclear cells in combination with laser tunneling of the muscles is most effective and can be recommended as a method of angiogenesis stimulation in non-reconstructable distal vascular pathology of the extremities .
	manualset3
249639	8	426546	16	NULL	NULL	0	NULL	muscles	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler sonography and immunofluorescence studies showed that intramuscular implantation of isolated fraction of autologous bone marrow mononuclear cells in combination with laser tunneling of the muscles is most effective and can be recommended as a method of angiogenesis stimulation in non-reconstructable distal vascular pathology of the extremities .
	manualset3
249640	9	426546	16	NULL	NULL	0	NULL	method	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler sonography and immunofluorescence studies showed that intramuscular implantation of isolated fraction of autologous bone marrow mononuclear cells in combination with laser tunneling of the muscles is most effective and can be recommended as a method of angiogenesis stimulation in non-reconstructable distal vascular pathology of the extremities .
	manualset3
249641	10	426546	16	NULL	NULL	0	NULL	angiogenesis stimulation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler sonography and immunofluorescence studies showed that intramuscular implantation of isolated fraction of autologous bone marrow mononuclear cells in combination with laser tunneling of the muscles is most effective and can be recommended as a method of angiogenesis stimulation in non-reconstructable distal vascular pathology of the extremities .
	manualset3
249642	11	426546	16	NULL	NULL	0	NULL	non-reconstructable distal vascular pathology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler sonography and immunofluorescence studies showed that intramuscular implantation of isolated fraction of autologous bone marrow mononuclear cells in combination with laser tunneling of the muscles is most effective and can be recommended as a method of angiogenesis stimulation in non-reconstructable distal vascular pathology of the extremities .
	manualset3
249643	12	426546	16	NULL	NULL	0	NULL	extremities	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler sonography and immunofluorescence studies showed that intramuscular implantation of isolated fraction of autologous bone marrow mononuclear cells in combination with laser tunneling of the muscles is most effective and can be recommended as a method of angiogenesis stimulation in non-reconstructable distal vascular pathology of the extremities .
	manualset3
249644	1	426547	16	NULL	NULL	0	NULL	Doppler ultrasonography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler ultrasonography of the middle cerebral artery was performed on 17 fetuses that were small for gestational age at the time of delivery .
	manualset3
249645	2	426547	16	NULL	NULL	0	NULL	middle cerebral artery	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler ultrasonography of the middle cerebral artery was performed on 17 fetuses that were small for gestational age at the time of delivery .
	manualset3
249646	3	426547	16	NULL	NULL	0	NULL	17 fetuses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler ultrasonography of the middle cerebral artery was performed on 17 fetuses that were small for gestational age at the time of delivery .
	manualset3
249647	4	426547	16	NULL	NULL	0	NULL	small	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler ultrasonography of the middle cerebral artery was performed on 17 fetuses that were small for gestational age at the time of delivery .
	manualset3
249648	5	426547	16	NULL	NULL	0	NULL	gestational age	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler ultrasonography of the middle cerebral artery was performed on 17 fetuses that were small for gestational age at the time of delivery .
	manualset3
249649	6	426547	16	NULL	NULL	0	NULL	time of delivery	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Doppler ultrasonography of the middle cerebral artery was performed on 17 fetuses that were small for gestational age at the time of delivery .
	manualset3
249650	1	426548	16	NULL	NULL	0	NULL	Dorsal periaqueductal gray-induced aversion	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dorsal periaqueductal gray-induced aversion as a simulation of panic anxiety : elements of face and predictive validity .
	manualset3
249651	2	426548	16	NULL	NULL	0	NULL	simulation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dorsal periaqueductal gray-induced aversion as a simulation of panic anxiety : elements of face and predictive validity .
	manualset3
249652	3	426548	16	NULL	NULL	0	NULL	panic anxiety	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dorsal periaqueductal gray-induced aversion as a simulation of panic anxiety : elements of face and predictive validity .
	manualset3
249653	4	426548	16	NULL	NULL	0	NULL	elements of face	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dorsal periaqueductal gray-induced aversion as a simulation of panic anxiety : elements of face and predictive validity .
	manualset3
249654	5	426548	16	NULL	NULL	0	NULL	predictive validity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dorsal periaqueductal gray-induced aversion as a simulation of panic anxiety : elements of face and predictive validity .
	manualset3
249655	1	426549	16	NULL	NULL	0	NULL	Dorsal blastomeres	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Dorsal blastomeres gave rise to trunk and tail structures containing dorsal mesoderm , whereas the ventral blastomere explants formed spheres containing solely ventral mesoderm .
	manualset3
249656	2	426549	16	NULL	NULL	0	NULL	rise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Dorsal blastomeres gave rise to trunk and tail structures containing dorsal mesoderm , whereas the ventral blastomere explants formed spheres containing solely ventral mesoderm .
	manualset3
249657	3	426549	16	NULL	NULL	0	NULL	trunk structures	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Dorsal blastomeres gave rise to trunk and tail structures containing dorsal mesoderm , whereas the ventral blastomere explants formed spheres containing solely ventral mesoderm .
	manualset3
249658	4	426549	16	NULL	NULL	0	NULL	tail structures	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Dorsal blastomeres gave rise to trunk and tail structures containing dorsal mesoderm , whereas the ventral blastomere explants formed spheres containing solely ventral mesoderm .
	manualset3
249659	5	426549	16	NULL	NULL	0	NULL	dorsal mesoderm	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Dorsal blastomeres gave rise to trunk and tail structures containing dorsal mesoderm , whereas the ventral blastomere explants formed spheres containing solely ventral mesoderm .
	manualset3
249660	6	426549	16	NULL	NULL	0	NULL	ventral blastomere explants	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Dorsal blastomeres gave rise to trunk and tail structures containing dorsal mesoderm , whereas the ventral blastomere explants formed spheres containing solely ventral mesoderm .
	manualset3
249661	7	426549	16	NULL	NULL	0	NULL	spheres	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dorsal blastomeres gave rise to trunk and tail structures containing dorsal mesoderm , whereas the ventral blastomere explants formed spheres containing solely ventral mesoderm .
	manualset3
249662	8	426549	16	NULL	NULL	0	NULL	ventral mesoderm	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Dorsal blastomeres gave rise to trunk and tail structures containing dorsal mesoderm , whereas the ventral blastomere explants formed spheres containing solely ventral mesoderm .
	manualset3
249767	1	426550	16	NULL	NULL	0	NULL	Dose-ranging study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose-ranging study of mometasone furoate dry powder inhaler in the treatment of moderate persistent asthma using fluticasone propionate as an active comparator .
	manualset3
249770	2	426550	16	NULL	NULL	0	NULL	mometasone furoate	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose-ranging study of mometasone furoate dry powder inhaler in the treatment of moderate persistent asthma using fluticasone propionate as an active comparator .
	manualset3
249772	3	426550	16	NULL	NULL	0	NULL	dry powder inhaler	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose-ranging study of mometasone furoate dry powder inhaler in the treatment of moderate persistent asthma using fluticasone propionate as an active comparator .
	manualset3
249774	4	426550	16	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose-ranging study of mometasone furoate dry powder inhaler in the treatment of moderate persistent asthma using fluticasone propionate as an active comparator .
	manualset3
249775	5	426550	16	NULL	NULL	0	NULL	moderate persistent asthma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose-ranging study of mometasone furoate dry powder inhaler in the treatment of moderate persistent asthma using fluticasone propionate as an active comparator .
	manualset3
249776	6	426550	16	NULL	NULL	0	NULL	fluticasone propionate	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose-ranging study of mometasone furoate dry powder inhaler in the treatment of moderate persistent asthma using fluticasone propionate as an active comparator .
	manualset3
249786	7	426550	16	NULL	NULL	0	NULL	active comparator	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose-ranging study of mometasone furoate dry powder inhaler in the treatment of moderate persistent asthma using fluticasone propionate as an active comparator .
	manualset3
249789	1	426551	16	NULL	NULL	0	NULL	Dose-response curves	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose-response curves indicated an apparent dissociation constant for the Cd blocking effect of 4.5 microM at 0 mV , with a one to one relationship between Cd and the slow channel .
	manualset3
249790	2	426551	16	NULL	NULL	0	NULL	dissociation constant	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose-response curves indicated an apparent dissociation constant for the Cd blocking effect of 4.5 microM at 0 mV , with a one to one relationship between Cd and the slow channel .
	manualset3
249791	3	426551	16	NULL	NULL	0	NULL	Cd blocking effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose-response curves indicated an apparent dissociation constant for the Cd blocking effect of 4.5 microM at 0 mV , with a one to one relationship between Cd and the slow channel .
	manualset3
249792	4	426551	16	NULL	NULL	0	NULL	4.5 microM at 0 mV	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose-response curves indicated an apparent dissociation constant for the Cd blocking effect of 4.5 microM at 0 mV , with a one to one relationship between Cd and the slow channel .
	manualset3
249793	5	426551	16	NULL	NULL	0	NULL	one to one relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose-response curves indicated an apparent dissociation constant for the Cd blocking effect of 4.5 microM at 0 mV , with a one to one relationship between Cd and the slow channel .
	manualset3
249794	6	426551	16	NULL	NULL	0	NULL	Cd	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose-response curves indicated an apparent dissociation constant for the Cd blocking effect of 4.5 microM at 0 mV , with a one to one relationship between Cd and the slow channel .
	manualset3
249795	7	426551	16	NULL	NULL	0	NULL	slow channel	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose-response curves indicated an apparent dissociation constant for the Cd blocking effect of 4.5 microM at 0 mV , with a one to one relationship between Cd and the slow channel .
	manualset3
249796	1	426552	16	NULL	NULL	0	NULL	Dose determination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose determination of cinacalcet hydrochloride in Japanese hemodialysis patients with secondary hyperparathyroidism .
	manualset3
249797	2	426552	16	NULL	NULL	0	NULL	cinacalcet hydrochloride	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose determination of cinacalcet hydrochloride in Japanese hemodialysis patients with secondary hyperparathyroidism .
	manualset3
249798	3	426552	16	NULL	NULL	0	NULL	Japanese hemodialysis patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose determination of cinacalcet hydrochloride in Japanese hemodialysis patients with secondary hyperparathyroidism .
	manualset3
249799	4	426552	16	NULL	NULL	0	NULL	secondary hyperparathyroidism	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose determination of cinacalcet hydrochloride in Japanese hemodialysis patients with secondary hyperparathyroidism .
	manualset3
249800	1	426553	16	NULL	NULL	0	NULL	Dose fractionation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose fractionation resulted in a significant increase of the survival , relative to that measured when X-ray dose was delivered in a single fraction .
	manualset3
249801	2	426553	16	NULL	NULL	0	NULL	increase	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose fractionation resulted in a significant increase of the survival , relative to that measured when X-ray dose was delivered in a single fraction .
	manualset3
249802	3	426553	16	NULL	NULL	0	NULL	survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose fractionation resulted in a significant increase of the survival , relative to that measured when X-ray dose was delivered in a single fraction .
	manualset3
249803	4	426553	16	NULL	NULL	0	NULL	relative	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose fractionation resulted in a significant increase of the survival , relative to that measured when X-ray dose was delivered in a single fraction .
	manualset3
249804	5	426553	16	NULL	NULL	0	NULL	X-ray dose	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose fractionation resulted in a significant increase of the survival , relative to that measured when X-ray dose was delivered in a single fraction .
	manualset3
249805	6	426553	16	NULL	NULL	0	NULL	single fraction	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose fractionation resulted in a significant increase of the survival , relative to that measured when X-ray dose was delivered in a single fraction .
	manualset3
249806	1	426554	16	NULL	NULL	NULL	NULL	Dose response	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dose response for spermatogonia treated with fractionated doses .
	manualset3
249807	2	426554	16	NULL	NULL	0	NULL	spermatogonia	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose response for spermatogonia treated with fractionated doses .
	manualset3
249808	3	426554	16	NULL	NULL	0	NULL	fractionated doses	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose response for spermatogonia treated with fractionated doses .
	manualset3
249809	1	426555	16	NULL	NULL	0	NULL	Dose response studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose response studies with both agonists demonstrated a direct relationship between the amount of thromboxane B2 produced and the amount of glutathione disulfide generated by stimulated platelets .
	manualset3
249810	2	426555	16	NULL	NULL	0	NULL	agonists	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose response studies with both agonists demonstrated a direct relationship between the amount of thromboxane B2 produced and the amount of glutathione disulfide generated by stimulated platelets .
	manualset3
249811	3	426555	16	NULL	NULL	0	NULL	direct relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose response studies with both agonists demonstrated a direct relationship between the amount of thromboxane B2 produced and the amount of glutathione disulfide generated by stimulated platelets .
	manualset3
249812	4	426555	16	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose response studies with both agonists demonstrated a direct relationship between the amount of thromboxane B2 produced and the amount of glutathione disulfide generated by stimulated platelets .
	manualset3
249813	5	426555	16	NULL	NULL	0	NULL	thromboxane B2	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose response studies with both agonists demonstrated a direct relationship between the amount of thromboxane B2 produced and the amount of glutathione disulfide generated by stimulated platelets .
	manualset3
249814	6	426555	16	NULL	NULL	0	NULL	amount	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose response studies with both agonists demonstrated a direct relationship between the amount of thromboxane B2 produced and the amount of glutathione disulfide generated by stimulated platelets .
	manualset3
249815	7	426555	16	NULL	NULL	0	NULL	glutathione disulfide	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose response studies with both agonists demonstrated a direct relationship between the amount of thromboxane B2 produced and the amount of glutathione disulfide generated by stimulated platelets .
	manualset3
249816	8	426555	16	NULL	NULL	0	NULL	stimulated platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Dose response studies with both agonists demonstrated a direct relationship between the amount of thromboxane B2 produced and the amount of glutathione disulfide generated by stimulated platelets .
	manualset3
249817	1	426556	16	NULL	NULL	0	NULL	Double-strength broth	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Double-strength broth was shown to be more reliable than the other two test methods , detecting the bacterial contaminants in 30 of 30 samples through six hours .
	manualset3
249818	2	426556	16	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Double-strength broth was shown to be more reliable than the other two test methods , detecting the bacterial contaminants in 30 of 30 samples through six hours .
	manualset3
249819	3	426556	16	NULL	NULL	0	NULL	test methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Double-strength broth was shown to be more reliable than the other two test methods , detecting the bacterial contaminants in 30 of 30 samples through six hours .
	manualset3
249820	4	426556	16	NULL	NULL	0	NULL	bacterial contaminants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Double-strength broth was shown to be more reliable than the other two test methods , detecting the bacterial contaminants in 30 of 30 samples through six hours .
	manualset3
249821	5	426556	16	NULL	NULL	0	NULL	30 of 30 samples	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Double-strength broth was shown to be more reliable than the other two test methods , detecting the bacterial contaminants in 30 of 30 samples through six hours .
	manualset3
249822	6	426556	16	NULL	NULL	0	NULL	six hours	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Double-strength broth was shown to be more reliable than the other two test methods , detecting the bacterial contaminants in 30 of 30 samples through six hours .
	manualset3
249823	1	426557	16	NULL	NULL	0	NULL	Double immunofluorescence	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Double immunofluorescence for heparanase and syndecan-3 revealed colocalization of the proteins in cell bodies of neurons and oligodendrocytes , suggestive of constitutive expression in these cell types .
	manualset3
249824	2	426557	16	NULL	NULL	0	NULL	heparanase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Double immunofluorescence for heparanase and syndecan-3 revealed colocalization of the proteins in cell bodies of neurons and oligodendrocytes , suggestive of constitutive expression in these cell types .
	manualset3
249825	3	426557	16	NULL	NULL	0	NULL	syndecan-3	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Double immunofluorescence for heparanase and syndecan-3 revealed colocalization of the proteins in cell bodies of neurons and oligodendrocytes , suggestive of constitutive expression in these cell types .
	manualset3
249826	4	426557	16	NULL	NULL	0	NULL	colocalization	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Double immunofluorescence for heparanase and syndecan-3 revealed colocalization of the proteins in cell bodies of neurons and oligodendrocytes , suggestive of constitutive expression in these cell types .
	manualset3
249827	5	426557	16	NULL	NULL	0	NULL	proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Double immunofluorescence for heparanase and syndecan-3 revealed colocalization of the proteins in cell bodies of neurons and oligodendrocytes , suggestive of constitutive expression in these cell types .
	manualset3
249828	6	426557	16	NULL	NULL	0	NULL	cell bodies	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Double immunofluorescence for heparanase and syndecan-3 revealed colocalization of the proteins in cell bodies of neurons and oligodendrocytes , suggestive of constitutive expression in these cell types .
	manualset3
249829	7	426557	16	NULL	NULL	0	NULL	neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Double immunofluorescence for heparanase and syndecan-3 revealed colocalization of the proteins in cell bodies of neurons and oligodendrocytes , suggestive of constitutive expression in these cell types .
	manualset3
249830	8	426557	16	NULL	NULL	0	NULL	oligodendrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Double immunofluorescence for heparanase and syndecan-3 revealed colocalization of the proteins in cell bodies of neurons and oligodendrocytes , suggestive of constitutive expression in these cell types .
	manualset3
249831	9	426557	16	NULL	NULL	0	NULL	constitutive expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Double immunofluorescence for heparanase and syndecan-3 revealed colocalization of the proteins in cell bodies of neurons and oligodendrocytes , suggestive of constitutive expression in these cell types .
	manualset3
249832	10	426557	16	NULL	NULL	0	NULL	cell types	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Double immunofluorescence for heparanase and syndecan-3 revealed colocalization of the proteins in cell bodies of neurons and oligodendrocytes , suggestive of constitutive expression in these cell types .
	manualset3
249833	1	426558	16	NULL	NULL	0	NULL	Double staining technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Double staining technique after colcemid treatment revealed that either keratin-positive or vimentin-positive cells were found with different ratios depending on the cases .
	manualset3
249834	2	426558	16	NULL	NULL	0	NULL	colcemid treatment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Double staining technique after colcemid treatment revealed that either keratin-positive or vimentin-positive cells were found with different ratios depending on the cases .
	manualset3
249835	3	426558	16	NULL	NULL	0	NULL	keratin-positive cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Double staining technique after colcemid treatment revealed that either keratin-positive or vimentin-positive cells were found with different ratios depending on the cases .
	manualset3
249836	4	426558	16	NULL	NULL	0	NULL	vimentin-positive cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Double staining technique after colcemid treatment revealed that either keratin-positive or vimentin-positive cells were found with different ratios depending on the cases .
	manualset3
249837	5	426558	16	NULL	NULL	0	NULL	ratios	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Double staining technique after colcemid treatment revealed that either keratin-positive or vimentin-positive cells were found with different ratios depending on the cases .
	manualset3
249838	6	426558	16	NULL	NULL	0	NULL	cases	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Double staining technique after colcemid treatment revealed that either keratin-positive or vimentin-positive cells were found with different ratios depending on the cases .
	manualset3
249839	1	426559	16	NULL	NULL	0	NULL	Doubly uniparental inheritance ( DUI )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Doubly uniparental inheritance ( DUI ) of mitochondrial ( mt ) DNA has been reported in the blue mussel Mytilus galloprovincialis .
	manualset3
249840	2	426559	16	NULL	NULL	0	NULL	mitochondrial ( mt ) DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Doubly uniparental inheritance ( DUI ) of mitochondrial ( mt ) DNA has been reported in the blue mussel Mytilus galloprovincialis .
	manualset3
249841	3	426559	16	NULL	NULL	0	NULL	blue mussel	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Doubly uniparental inheritance ( DUI ) of mitochondrial ( mt ) DNA has been reported in the blue mussel Mytilus galloprovincialis .
	manualset3
249842	4	426559	16	NULL	NULL	0	NULL	Mytilus galloprovincialis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Doubly uniparental inheritance ( DUI ) of mitochondrial ( mt ) DNA has been reported in the blue mussel Mytilus galloprovincialis .
	manualset3
249843	1	426560	16	NULL	NULL	0	NULL	repercussion	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Doubt to the repercussion that the ICP values have on clinical evolutions we conclude that the nurse has to respond in an efficient , early and autonomous way in order to avoid uncontrolled elevation of ICP values during habitual management of patient .
	manualset3
249844	2	426560	16	NULL	NULL	0	NULL	ICP values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Doubt to the repercussion that the ICP values have on clinical evolutions we conclude that the nurse has to respond in an efficient , early and autonomous way in order to avoid uncontrolled elevation of ICP values during habitual management of patient .
	manualset3
249845	3	426560	16	NULL	NULL	0	NULL	clinical evolutions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Doubt to the repercussion that the ICP values have on clinical evolutions we conclude that the nurse has to respond in an efficient , early and autonomous way in order to avoid uncontrolled elevation of ICP values during habitual management of patient .
	manualset3
249846	4	426560	16	NULL	NULL	0	NULL	nurse	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Doubt to the repercussion that the ICP values have on clinical evolutions we conclude that the nurse has to respond in an efficient , early and autonomous way in order to avoid uncontrolled elevation of ICP values during habitual management of patient .
	manualset3
249847	5	426560	16	NULL	NULL	0	NULL	autonomous way	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Doubt to the repercussion that the ICP values have on clinical evolutions we conclude that the nurse has to respond in an efficient , early and autonomous way in order to avoid uncontrolled elevation of ICP values during habitual management of patient .
	manualset3
249848	6	426560	16	NULL	NULL	0	NULL	elevation	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Doubt to the repercussion that the ICP values have on clinical evolutions we conclude that the nurse has to respond in an efficient , early and autonomous way in order to avoid uncontrolled elevation of ICP values during habitual management of patient .
	manualset3
249849	7	426560	16	NULL	NULL	0	NULL	ICP values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Doubt to the repercussion that the ICP values have on clinical evolutions we conclude that the nurse has to respond in an efficient , early and autonomous way in order to avoid uncontrolled elevation of ICP values during habitual management of patient .
	manualset3
249850	8	426560	16	NULL	NULL	0	NULL	habitual management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Doubt to the repercussion that the ICP values have on clinical evolutions we conclude that the nurse has to respond in an efficient , early and autonomous way in order to avoid uncontrolled elevation of ICP values during habitual management of patient .
	manualset3
249851	9	426560	16	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Doubt to the repercussion that the ICP values have on clinical evolutions we conclude that the nurse has to respond in an efficient , early and autonomous way in order to avoid uncontrolled elevation of ICP values during habitual management of patient .
	manualset3
249852	1	426561	16	NULL	NULL	0	NULL	nomenclature	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the nomenclature and classification of toxemia ) .
	manualset3
249853	2	426561	16	NULL	NULL	0	NULL	classification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the nomenclature and classification of toxemia ) .
	manualset3
249854	3	426561	16	NULL	NULL	0	NULL	toxemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the nomenclature and classification of toxemia ) .
	manualset3
249855	1	426562	16	NULL	NULL	0	NULL	Doubtful value	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Doubtful value of bicuculline as a specific antagonist of GABA .
	manualset3
249856	2	426562	16	NULL	NULL	0	NULL	bicuculline	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Doubtful value of bicuculline as a specific antagonist of GABA .
	manualset3
249857	3	426562	16	NULL	NULL	0	NULL	specific antagonist	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Doubtful value of bicuculline as a specific antagonist of GABA .
	manualset3
249858	4	426562	16	NULL	NULL	NULL	NULL	GABA	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Doubtful value of bicuculline as a specific antagonist of GABA .
	manualset3
249859	1	426563	16	NULL	NULL	0	NULL	Doubts	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Doubts about its efficacy and mechanism of action prompted us to evaluate the immunological changes that occurred in a group of 99 patients selected for their confirmed allergic sensitivity to house dust , and who showed significant clinical improvement after a minimum of 12 months of immunotherapy with HDE .
	manualset3
249860	2	426563	16	NULL	NULL	0	NULL	efficacy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Doubts about its efficacy and mechanism of action prompted us to evaluate the immunological changes that occurred in a group of 99 patients selected for their confirmed allergic sensitivity to house dust , and who showed significant clinical improvement after a minimum of 12 months of immunotherapy with HDE .
	manualset3
249861	3	426563	16	NULL	NULL	0	NULL	mechanism of action	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Doubts about its efficacy and mechanism of action prompted us to evaluate the immunological changes that occurred in a group of 99 patients selected for their confirmed allergic sensitivity to house dust , and who showed significant clinical improvement after a minimum of 12 months of immunotherapy with HDE .
	manualset3
249862	4	426563	16	NULL	NULL	0	NULL	immunological changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Doubts about its efficacy and mechanism of action prompted us to evaluate the immunological changes that occurred in a group of 99 patients selected for their confirmed allergic sensitivity to house dust , and who showed significant clinical improvement after a minimum of 12 months of immunotherapy with HDE .
	manualset3
249863	5	426563	16	NULL	NULL	0	NULL	group of 99 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Doubts about its efficacy and mechanism of action prompted us to evaluate the immunological changes that occurred in a group of 99 patients selected for their confirmed allergic sensitivity to house dust , and who showed significant clinical improvement after a minimum of 12 months of immunotherapy with HDE .
	manualset3
249864	6	426563	16	NULL	NULL	0	NULL	allergic sensitivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Doubts about its efficacy and mechanism of action prompted us to evaluate the immunological changes that occurred in a group of 99 patients selected for their confirmed allergic sensitivity to house dust , and who showed significant clinical improvement after a minimum of 12 months of immunotherapy with HDE .
	manualset3
249865	7	426563	16	NULL	NULL	0	NULL	house dust	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Doubts about its efficacy and mechanism of action prompted us to evaluate the immunological changes that occurred in a group of 99 patients selected for their confirmed allergic sensitivity to house dust , and who showed significant clinical improvement after a minimum of 12 months of immunotherapy with HDE .
	manualset3
249866	8	426563	16	NULL	NULL	0	NULL	clinical improvement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Doubts about its efficacy and mechanism of action prompted us to evaluate the immunological changes that occurred in a group of 99 patients selected for their confirmed allergic sensitivity to house dust , and who showed significant clinical improvement after a minimum of 12 months of immunotherapy with HDE .
	manualset3
249867	9	426563	16	NULL	NULL	0	NULL	12 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Doubts about its efficacy and mechanism of action prompted us to evaluate the immunological changes that occurred in a group of 99 patients selected for their confirmed allergic sensitivity to house dust , and who showed significant clinical improvement after a minimum of 12 months of immunotherapy with HDE .
	manualset3
249868	10	426563	16	NULL	NULL	0	NULL	immunotherapy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Doubts about its efficacy and mechanism of action prompted us to evaluate the immunological changes that occurred in a group of 99 patients selected for their confirmed allergic sensitivity to house dust , and who showed significant clinical improvement after a minimum of 12 months of immunotherapy with HDE .
	manualset3
249869	11	426563	16	NULL	NULL	0	NULL	HDE	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Doubts about its efficacy and mechanism of action prompted us to evaluate the immunological changes that occurred in a group of 99 patients selected for their confirmed allergic sensitivity to house dust , and who showed significant clinical improvement after a minimum of 12 months of immunotherapy with HDE .
	manualset3
250214	1	426564	16	NULL	NULL	0	NULL	Down-regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Down-regulation of actin genes precedes microfilament network disruption and actin cleavage during p53-mediated apoptosis .
	manualset3
250215	2	426564	16	NULL	NULL	0	NULL	actin genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Down-regulation of actin genes precedes microfilament network disruption and actin cleavage during p53-mediated apoptosis .
	manualset3
250216	3	426564	16	NULL	NULL	0	NULL	microfilament network disruption	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Down-regulation of actin genes precedes microfilament network disruption and actin cleavage during p53-mediated apoptosis .
	manualset3
250217	4	426564	16	NULL	NULL	0	NULL	actin cleavage	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Down-regulation of actin genes precedes microfilament network disruption and actin cleavage during p53-mediated apoptosis .
	manualset3
250218	5	426564	16	NULL	NULL	0	NULL	p53-mediated apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Down-regulation of actin genes precedes microfilament network disruption and actin cleavage during p53-mediated apoptosis .
	manualset3
250220	1	426565	16	NULL	NULL	0	NULL	Down-regulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Down-regulation of apurinic/apyrimidinic endonuclease expression is associated with the induction of apoptosis in differentiating myeloid leukemia cells .
	manualset3
250221	2	426565	16	NULL	NULL	0	NULL	apurinic/apyrimidinic endonuclease expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Down-regulation of apurinic/apyrimidinic endonuclease expression is associated with the induction of apoptosis in differentiating myeloid leukemia cells .
	manualset3
250222	3	426565	16	NULL	NULL	0	NULL	induction of apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Down-regulation of apurinic/apyrimidinic endonuclease expression is associated with the induction of apoptosis in differentiating myeloid leukemia cells .
	manualset3
250223	4	426565	16	NULL	NULL	0	NULL	myeloid leukemia cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Down-regulation of apurinic/apyrimidinic endonuclease expression is associated with the induction of apoptosis in differentiating myeloid leukemia cells .
	manualset3
250224	1	426566	16	NULL	NULL	0	NULL	Downregulation of FAK-related non-kinase	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Downregulation of FAK-related non-kinase mediates the migratory phenotype of human fibrotic lung fibroblasts .
	manualset3
250226	2	426566	16	NULL	NULL	0	NULL	migratory phenotype	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Downregulation of FAK-related non-kinase mediates the migratory phenotype of human fibrotic lung fibroblasts .
	manualset3
250230	3	426566	16	NULL	NULL	0	NULL	human fibrotic lung fibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Downregulation of FAK-related non-kinase mediates the migratory phenotype of human fibrotic lung fibroblasts .
	manualset3
250240	1	426567	16	NULL	NULL	0	NULL	Downregulation of nitric oxide accumulation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Downregulation of nitric oxide accumulation by cyclooxygenase-2 induction and thromboxane A2 production in interleukin-1beta-stimulated rat aortic smooth muscle cells .
	manualset3
250241	2	426567	16	NULL	NULL	0	NULL	cyclooxygenase-2 induction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Downregulation of nitric oxide accumulation by cyclooxygenase-2 induction and thromboxane A2 production in interleukin-1beta-stimulated rat aortic smooth muscle cells .
	manualset3
250242	3	426567	16	NULL	NULL	0	NULL	thromboxane A2 production	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Downregulation of nitric oxide accumulation by cyclooxygenase-2 induction and thromboxane A2 production in interleukin-1beta-stimulated rat aortic smooth muscle cells .
	manualset3
250243	4	426567	16	NULL	NULL	0	NULL	 interleukin-1beta	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Downregulation of nitric oxide accumulation by cyclooxygenase-2 induction and thromboxane A2 production in interleukin-1beta-stimulated rat aortic smooth muscle cells .
	manualset3
250244	5	426567	16	NULL	NULL	0	NULL	rat aortic smooth muscle cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Downregulation of nitric oxide accumulation by cyclooxygenase-2 induction and thromboxane A2 production in interleukin-1beta-stimulated rat aortic smooth muscle cells .
	manualset3
250245	1	426568	16	NULL	NULL	0	NULL	Doxorubicin	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Doxorubicin and vinorelbine act independently via p53 expression and p38 activation respectively in breast cancer cell lines .
	manualset3
250246	2	426568	16	NULL	NULL	0	NULL	vinorelbine	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Doxorubicin and vinorelbine act independently via p53 expression and p38 activation respectively in breast cancer cell lines .
	manualset3
250247	3	426568	16	NULL	NULL	0	NULL	p53 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Doxorubicin and vinorelbine act independently via p53 expression and p38 activation respectively in breast cancer cell lines .
	manualset3
250248	4	426568	16	NULL	NULL	0	NULL	p38 activation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Doxorubicin and vinorelbine act independently via p53 expression and p38 activation respectively in breast cancer cell lines .
	manualset3
250249	5	426568	16	NULL	NULL	0	NULL	breast cancer cell lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Doxorubicin and vinorelbine act independently via p53 expression and p38 activation respectively in breast cancer cell lines .
	manualset3
250250	1	426569	16	NULL	NULL	0	NULL	Doxorubicin 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Doxorubicin is one of the most effective molecules used in the treatment of various tumors .
	manualset3
250251	2	426569	16	NULL	NULL	0	NULL	effective molecules	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Doxorubicin is one of the most effective molecules used in the treatment of various tumors .
	manualset3
250252	3	426569	16	NULL	NULL	0	NULL	 treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Doxorubicin is one of the most effective molecules used in the treatment of various tumors .
	manualset3
250253	4	426569	16	NULL	NULL	0	NULL	tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Doxorubicin is one of the most effective molecules used in the treatment of various tumors .
	manualset3
250254	1	426570	16	NULL	NULL	0	NULL	Dr. Best	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Dr. Best , insulin , and molecular evolution .
	manualset3
250255	2	426570	16	NULL	NULL	0	NULL	 insulin	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	Dr. Best , insulin , and molecular evolution .
	manualset3
250256	3	426570	16	NULL	NULL	0	NULL	molecular evolution	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dr. Best , insulin , and molecular evolution .
	manualset3
250257	1	426571	16	NULL	NULL	0	NULL	 origin therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the origin therapy and rehabilitation of involution psychosis ) .
	manualset3
250258	2	426571	16	NULL	NULL	0	NULL	rehabilitation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the origin therapy and rehabilitation of involution psychosis ) .
	manualset3
250259	3	426571	16	NULL	NULL	0	NULL	involution psychosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the origin therapy and rehabilitation of involution psychosis ) .
	manualset3
250260	1	426572	16	NULL	NULL	0	NULL	Drainage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Drainage of esophageal leakage using endoscopic vacuum therapy : a prospective pilot study .
	manualset3
250261	2	426572	16	NULL	NULL	0	NULL	esophageal leakage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Drainage of esophageal leakage using endoscopic vacuum therapy : a prospective pilot study .
	manualset3
250262	3	426572	16	NULL	NULL	0	NULL	endoscopic vacuum therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Drainage of esophageal leakage using endoscopic vacuum therapy : a prospective pilot study .
	manualset3
250263	4	426572	16	NULL	NULL	0	NULL	prospective pilot study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Drainage of esophageal leakage using endoscopic vacuum therapy : a prospective pilot study .
	manualset3
250264	1	426573	16	NULL	NULL	0	NULL	Drak2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Drak2 is a serine threonine kinase in the death-associated protein family .
	manualset3
250265	2	426573	16	NULL	NULL	0	NULL	serine threonine kinase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Drak2 is a serine threonine kinase in the death-associated protein family .
	manualset3
250266	3	426573	16	NULL	NULL	0	NULL	death-associated protein family	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Drak2 is a serine threonine kinase in the death-associated protein family .
	manualset3
250285	1	426574	16	NULL	NULL	0	NULL	differences	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Dramatic differences between the energy landscapes of SiO ( 2 ) and SiS ( 2 ) zeotype materials .
	manualset3
250287	2	426574	16	NULL	NULL	0	NULL	energy landscapes	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Dramatic differences between the energy landscapes of SiO ( 2 ) and SiS ( 2 ) zeotype materials .
	manualset3
250288	3	426574	16	NULL	NULL	0	NULL	SiO ( 2 ) zeotype materials	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Dramatic differences between the energy landscapes of SiO ( 2 ) and SiS ( 2 ) zeotype materials .
	manualset3
250289	4	426574	16	NULL	NULL	0	NULL	SiS ( 2 ) zeotype materials	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Dramatic differences between the energy landscapes of SiO ( 2 ) and SiS ( 2 ) zeotype materials .
	manualset3
250290	1	426575	16	NULL	NULL	NULL	NULL	gains	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Drive further gains in workforce productivity through return to work strategy .
	manualset3
250291	2	426575	16	NULL	NULL	0	NULL	workforce productivity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Drive further gains in workforce productivity through return to work strategy .
	manualset3
250293	3	426575	16	NULL	NULL	0	NULL	return to work strategy	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Drive further gains in workforce productivity through return to work strategy .
	manualset3
250297	1	426576	16	NULL	NULL	0	NULL	Drug-induced contraction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug-induced contraction of gastrointestinal tracts seems to depend upon the extent of their rhythmic contraction that is driven by the activity of gastrointestinal pacemaker cells .
	manualset3
250298	2	426576	16	NULL	NULL	0	NULL	gastrointestinal tracts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug-induced contraction of gastrointestinal tracts seems to depend upon the extent of their rhythmic contraction that is driven by the activity of gastrointestinal pacemaker cells .
	manualset3
250299	3	426576	16	NULL	NULL	0	NULL	extent	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug-induced contraction of gastrointestinal tracts seems to depend upon the extent of their rhythmic contraction that is driven by the activity of gastrointestinal pacemaker cells .
	manualset3
250300	4	426576	16	NULL	NULL	0	NULL	rhythmic contraction	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug-induced contraction of gastrointestinal tracts seems to depend upon the extent of their rhythmic contraction that is driven by the activity of gastrointestinal pacemaker cells .
	manualset3
250301	5	426576	16	NULL	NULL	0	NULL	activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug-induced contraction of gastrointestinal tracts seems to depend upon the extent of their rhythmic contraction that is driven by the activity of gastrointestinal pacemaker cells .
	manualset3
250302	6	426576	16	NULL	NULL	0	NULL	gastrointestinal pacemaker cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug-induced contraction of gastrointestinal tracts seems to depend upon the extent of their rhythmic contraction that is driven by the activity of gastrointestinal pacemaker cells .
	manualset3
250303	1	426577	16	NULL	NULL	NULL	NULL	Drug-induced interstitial lung disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Drug-induced interstitial lung disease should be remembered as a possible complication of anticonvulsant treatment , such as VPA and ZNS .
	manualset3
250304	2	426577	16	NULL	NULL	0	NULL	complication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug-induced interstitial lung disease should be remembered as a possible complication of anticonvulsant treatment , such as VPA and ZNS .
	manualset3
250305	3	426577	16	NULL	NULL	0	NULL	 anticonvulsant treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug-induced interstitial lung disease should be remembered as a possible complication of anticonvulsant treatment , such as VPA and ZNS .
	manualset3
250306	4	426577	16	NULL	NULL	0	NULL	VPA	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug-induced interstitial lung disease should be remembered as a possible complication of anticonvulsant treatment , such as VPA and ZNS .
	manualset3
250307	5	426577	16	NULL	NULL	0	NULL	ZNS	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug-induced interstitial lung disease should be remembered as a possible complication of anticonvulsant treatment , such as VPA and ZNS .
	manualset3
250308	1	426578	16	NULL	NULL	0	NULL	Drug-like inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug-like inhibitors of IL-2 have been identified through a combination of fragment discovery , structure-based design , and medicinal chemistry ; this discovery approach illustrates the importance of using a diverse range of complementary screening methods and analytical tools to achieve a comprehensive understanding of molecular recognition .
	manualset3
250309	2	426578	16	NULL	NULL	0	NULL	IL-2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug-like inhibitors of IL-2 have been identified through a combination of fragment discovery , structure-based design , and medicinal chemistry ; this discovery approach illustrates the importance of using a diverse range of complementary screening methods and analytical tools to achieve a comprehensive understanding of molecular recognition .
	manualset3
250311	4	426578	16	NULL	NULL	0	NULL	combination	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug-like inhibitors of IL-2 have been identified through a combination of fragment discovery , structure-based design , and medicinal chemistry ; this discovery approach illustrates the importance of using a diverse range of complementary screening methods and analytical tools to achieve a comprehensive understanding of molecular recognition .
	manualset3
250312	5	426578	16	NULL	NULL	0	NULL	fragment discovery	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug-like inhibitors of IL-2 have been identified through a combination of fragment discovery , structure-based design , and medicinal chemistry ; this discovery approach illustrates the importance of using a diverse range of complementary screening methods and analytical tools to achieve a comprehensive understanding of molecular recognition .
	manualset3
250313	6	426578	16	NULL	NULL	0	NULL	structure-based design	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug-like inhibitors of IL-2 have been identified through a combination of fragment discovery , structure-based design , and medicinal chemistry ; this discovery approach illustrates the importance of using a diverse range of complementary screening methods and analytical tools to achieve a comprehensive understanding of molecular recognition .
	manualset3
250314	7	426578	16	NULL	NULL	0	NULL	medicinal chemistry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug-like inhibitors of IL-2 have been identified through a combination of fragment discovery , structure-based design , and medicinal chemistry ; this discovery approach illustrates the importance of using a diverse range of complementary screening methods and analytical tools to achieve a comprehensive understanding of molecular recognition .
	manualset3
250315	8	426578	16	NULL	NULL	0	NULL	discovery approach	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug-like inhibitors of IL-2 have been identified through a combination of fragment discovery , structure-based design , and medicinal chemistry ; this discovery approach illustrates the importance of using a diverse range of complementary screening methods and analytical tools to achieve a comprehensive understanding of molecular recognition .
	manualset3
250316	9	426578	16	NULL	NULL	0	NULL	importance	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug-like inhibitors of IL-2 have been identified through a combination of fragment discovery , structure-based design , and medicinal chemistry ; this discovery approach illustrates the importance of using a diverse range of complementary screening methods and analytical tools to achieve a comprehensive understanding of molecular recognition .
	manualset3
250317	10	426578	16	NULL	NULL	0	NULL	range	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug-like inhibitors of IL-2 have been identified through a combination of fragment discovery , structure-based design , and medicinal chemistry ; this discovery approach illustrates the importance of using a diverse range of complementary screening methods and analytical tools to achieve a comprehensive understanding of molecular recognition .
	manualset3
250318	11	426578	16	NULL	NULL	0	NULL	screening methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug-like inhibitors of IL-2 have been identified through a combination of fragment discovery , structure-based design , and medicinal chemistry ; this discovery approach illustrates the importance of using a diverse range of complementary screening methods and analytical tools to achieve a comprehensive understanding of molecular recognition .
	manualset3
250319	12	426578	16	NULL	NULL	0	NULL	analytical tools	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug-like inhibitors of IL-2 have been identified through a combination of fragment discovery , structure-based design , and medicinal chemistry ; this discovery approach illustrates the importance of using a diverse range of complementary screening methods and analytical tools to achieve a comprehensive understanding of molecular recognition .
	manualset3
250320	13	426578	16	NULL	NULL	0	NULL	understanding	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug-like inhibitors of IL-2 have been identified through a combination of fragment discovery , structure-based design , and medicinal chemistry ; this discovery approach illustrates the importance of using a diverse range of complementary screening methods and analytical tools to achieve a comprehensive understanding of molecular recognition .
	manualset3
250321	1	426579	16	NULL	NULL	0	NULL	Drug-resistant TB	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug-resistant TB may bring epidemic .
	manualset3
250322	2	426579	16	NULL	NULL	0	NULL	epidemic	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug-resistant TB may bring epidemic .
	manualset3
250323	1	426580	16	NULL	NULL	0	NULL	Drug targeting	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug targeting Mycobacterium tuberculosis cell wall synthesis : genetics of dTDP-rhamnose synthetic enzymes and development of a microtiter plate-based screen for inhibitors of conversion of dTDP-glucose to dTDP-rhamnose .
	manualset3
250324	2	426580	16	NULL	NULL	0	NULL	Mycobacterium tuberculosis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug targeting Mycobacterium tuberculosis cell wall synthesis : genetics of dTDP-rhamnose synthetic enzymes and development of a microtiter plate-based screen for inhibitors of conversion of dTDP-glucose to dTDP-rhamnose .
	manualset3
250325	3	426580	16	NULL	NULL	0	NULL	cell wall synthesis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug targeting Mycobacterium tuberculosis cell wall synthesis : genetics of dTDP-rhamnose synthetic enzymes and development of a microtiter plate-based screen for inhibitors of conversion of dTDP-glucose to dTDP-rhamnose .
	manualset3
250326	4	426580	16	NULL	NULL	0	NULL	genetics	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug targeting Mycobacterium tuberculosis cell wall synthesis : genetics of dTDP-rhamnose synthetic enzymes and development of a microtiter plate-based screen for inhibitors of conversion of dTDP-glucose to dTDP-rhamnose .
	manualset3
250327	5	426580	16	NULL	NULL	0	NULL	dTDP-rhamnose synthetic enzymes	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug targeting Mycobacterium tuberculosis cell wall synthesis : genetics of dTDP-rhamnose synthetic enzymes and development of a microtiter plate-based screen for inhibitors of conversion of dTDP-glucose to dTDP-rhamnose .
	manualset3
250328	6	426580	16	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug targeting Mycobacterium tuberculosis cell wall synthesis : genetics of dTDP-rhamnose synthetic enzymes and development of a microtiter plate-based screen for inhibitors of conversion of dTDP-glucose to dTDP-rhamnose .
	manualset3
250329	7	426580	16	NULL	NULL	NULL	NULL	microtiter plate-based screen	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Drug targeting Mycobacterium tuberculosis cell wall synthesis : genetics of dTDP-rhamnose synthetic enzymes and development of a microtiter plate-based screen for inhibitors of conversion of dTDP-glucose to dTDP-rhamnose .
	manualset3
250330	8	426580	16	NULL	NULL	0	NULL	inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug targeting Mycobacterium tuberculosis cell wall synthesis : genetics of dTDP-rhamnose synthetic enzymes and development of a microtiter plate-based screen for inhibitors of conversion of dTDP-glucose to dTDP-rhamnose .
	manualset3
250331	9	426580	16	NULL	NULL	0	NULL	conversion of dTDP-glucose to dTDP-rhamnose	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug targeting Mycobacterium tuberculosis cell wall synthesis : genetics of dTDP-rhamnose synthetic enzymes and development of a microtiter plate-based screen for inhibitors of conversion of dTDP-glucose to dTDP-rhamnose .
	manualset3
250332	1	426581	16	NULL	NULL	0	NULL	Drug excipients compatibility studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug excipients compatibility studies demonstrated no interaction between drug and polymer .
	manualset3
250333	2	426581	16	NULL	NULL	0	NULL	interaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug excipients compatibility studies demonstrated no interaction between drug and polymer .
	manualset3
250334	3	426581	16	NULL	NULL	0	NULL	drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug excipients compatibility studies demonstrated no interaction between drug and polymer .
	manualset3
250335	4	426581	16	NULL	NULL	0	NULL	polymer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug excipients compatibility studies demonstrated no interaction between drug and polymer .
	manualset3
250336	1	426582	16	NULL	NULL	0	NULL	Drug charcoal slurries	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug charcoal slurries were vortex-mixed , centrifuged and analyzed for free drug .
	manualset3
250337	2	426582	16	NULL	NULL	0	NULL	free drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug charcoal slurries were vortex-mixed , centrifuged and analyzed for free drug .
	manualset3
250338	1	426583	16	NULL	NULL	0	NULL	Drug concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug concentrations were seen to change following storage , the greatest changes occurring with the highly lipophilic drugs dexamethasone and diazepam .
	manualset3
250339	2	426583	16	NULL	NULL	0	NULL	storage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug concentrations were seen to change following storage , the greatest changes occurring with the highly lipophilic drugs dexamethasone and diazepam .
	manualset3
250340	3	426583	16	NULL	NULL	0	NULL	changes	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug concentrations were seen to change following storage , the greatest changes occurring with the highly lipophilic drugs dexamethasone and diazepam .
	manualset3
250341	4	426583	16	NULL	NULL	0	NULL	lipophilic drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug concentrations were seen to change following storage , the greatest changes occurring with the highly lipophilic drugs dexamethasone and diazepam .
	manualset3
250342	5	426583	16	NULL	NULL	0	NULL	dexamethasone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug concentrations were seen to change following storage , the greatest changes occurring with the highly lipophilic drugs dexamethasone and diazepam .
	manualset3
250343	6	426583	16	NULL	NULL	0	NULL	diazepam	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug concentrations were seen to change following storage , the greatest changes occurring with the highly lipophilic drugs dexamethasone and diazepam .
	manualset3
250344	1	426584	16	NULL	NULL	0	NULL	Drug development	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug development for children : how is pharma tackling an unmet need ?
	manualset3
250345	2	426584	16	NULL	NULL	0	NULL	children	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug development for children : how is pharma tackling an unmet need ?
	manualset3
250346	3	426584	16	NULL	NULL	0	NULL	pharma	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug development for children : how is pharma tackling an unmet need ?
	manualset3
250347	4	426584	16	NULL	NULL	0	NULL	unmet need	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug development for children : how is pharma tackling an unmet need ?
	manualset3
250348	1	426585	16	NULL	NULL	0	NULL	Drug resistance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug resistance in M. tuberculosis is caused by mutations in restricted regions of the genome .
	manualset3
250349	2	426585	16	NULL	NULL	0	NULL	M. tuberculosis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug resistance in M. tuberculosis is caused by mutations in restricted regions of the genome .
	manualset3
250350	3	426585	16	NULL	NULL	0	NULL	mutations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug resistance in M. tuberculosis is caused by mutations in restricted regions of the genome .
	manualset3
250351	4	426585	16	NULL	NULL	0	NULL	restricted regions	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug resistance in M. tuberculosis is caused by mutations in restricted regions of the genome .
	manualset3
250352	5	426585	16	NULL	NULL	0	NULL	genome	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug resistance in M. tuberculosis is caused by mutations in restricted regions of the genome .
	manualset3
250930	1	426586	16	NULL	NULL	NULL	NULL	Drug resistance strategies	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Drug resistance strategies and substance use among adolescents in Monterrey , Mexico .
	manualset3
250932	3	426586	16	NULL	NULL	0	NULL	substance use	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug resistance strategies and substance use among adolescents in Monterrey , Mexico .
	manualset3
250933	4	426586	16	NULL	NULL	0	NULL	adolescents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug resistance strategies and substance use among adolescents in Monterrey , Mexico .
	manualset3
250934	5	426586	16	NULL	NULL	0	NULL	Monterrey	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug resistance strategies and substance use among adolescents in Monterrey , Mexico .
	manualset3
250935	6	426586	16	NULL	NULL	0	NULL	Mexico	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug resistance strategies and substance use among adolescents in Monterrey , Mexico .
	manualset3
250924	1	426587	16	NULL	NULL	0	NULL	Drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug shortages in health care institutions : perspectives in early 2012 .
	manualset3
250925	2	426587	16	NULL	NULL	0	NULL	shortages	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug shortages in health care institutions : perspectives in early 2012 .
	manualset3
250926	3	426587	16	NULL	NULL	0	NULL	health care institutions	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug shortages in health care institutions : perspectives in early 2012 .
	manualset3
250936	4	426587	16	NULL	NULL	0	NULL	perspectives	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug shortages in health care institutions : perspectives in early 2012 .
	manualset3
250937	5	426587	16	NULL	NULL	0	NULL	2012	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug shortages in health care institutions : perspectives in early 2012 .
	manualset3
250938	1	426588	16	NULL	NULL	0	NULL	Drug solubilization effect	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug solubilization effect of lauroyl-L-glutamate .
	manualset3
250939	2	426588	16	NULL	NULL	0	NULL	lauroyl-L-glutamate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug solubilization effect of lauroyl-L-glutamate .
	manualset3
250940	1	426589	16	NULL	NULL	0	NULL	preoperative importance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the preoperative and postoperative importance of dye dilution curves in auricular septal defect ) .
	manualset3
250941	2	426589	16	NULL	NULL	0	NULL	postoperative importance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the preoperative and postoperative importance of dye dilution curves in auricular septal defect ) .
	manualset3
250942	3	426589	16	NULL	NULL	0	NULL	dye dilution curves	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the preoperative and postoperative importance of dye dilution curves in auricular septal defect ) .
	manualset3
250943	4	426589	16	NULL	NULL	0	NULL	auricular septal defect	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the preoperative and postoperative importance of dye dilution curves in auricular septal defect ) .
	manualset3
250944	1	426590	16	NULL	NULL	0	NULL	Drug use	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug use and four kinds of novelty-seeking .
	manualset3
250945	2	426590	16	NULL	NULL	0	NULL	four	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug use and four kinds of novelty-seeking .
	manualset3
250946	3	426590	16	NULL	NULL	0	NULL	novelty-seeking	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Drug use and four kinds of novelty-seeking .
	manualset3
250947	1	426591	16	NULL	NULL	0	NULL	Drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Drugs for neuromuscular pain and spasm .
	manualset3
250948	2	426591	16	NULL	NULL	0	NULL	neuromuscular pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Drugs for neuromuscular pain and spasm .
	manualset3
250949	3	426591	16	NULL	NULL	0	NULL	neuromuscular spasm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Drugs for neuromuscular pain and spasm .
	manualset3
250950	1	426592	16	NULL	NULL	0	NULL	Drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Drugs that enhance brain serotonergic activity reduced p , p ' - DDT-induced myoclonus , and serotonin antagonists invariably aggravated this syndrome .
	manualset3
250951	2	426592	16	NULL	NULL	NULL	NULL	brain serotonergic activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Drugs that enhance brain serotonergic activity reduced p , p ' - DDT-induced myoclonus , and serotonin antagonists invariably aggravated this syndrome .
	manualset3
250952	3	426592	16	NULL	NULL	0	NULL	p , p ' - DDT-induced myoclonus	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Drugs that enhance brain serotonergic activity reduced p , p ' - DDT-induced myoclonus , and serotonin antagonists invariably aggravated this syndrome .
	manualset3
250953	4	426592	16	NULL	NULL	0	NULL	serotonin antagonists	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Drugs that enhance brain serotonergic activity reduced p , p ' - DDT-induced myoclonus , and serotonin antagonists invariably aggravated this syndrome .
	manualset3
250954	5	426592	16	NULL	NULL	0	NULL	syndrome	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Drugs that enhance brain serotonergic activity reduced p , p ' - DDT-induced myoclonus , and serotonin antagonists invariably aggravated this syndrome .
	manualset3
250955	1	426593	16	NULL	NULL	0	NULL	Drusen	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Drusen contained cores , basally located regions that were intensely bright when stained for UC or deeply dark when stained for EC ; many were surrounded by concentric lamellae .
	manualset3
250956	2	426593	16	NULL	NULL	0	NULL	cores	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Drusen contained cores , basally located regions that were intensely bright when stained for UC or deeply dark when stained for EC ; many were surrounded by concentric lamellae .
	manualset3
250957	3	426593	16	NULL	NULL	0	NULL	regions	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Drusen contained cores , basally located regions that were intensely bright when stained for UC or deeply dark when stained for EC ; many were surrounded by concentric lamellae .
	manualset3
250958	4	426593	16	NULL	NULL	0	NULL	UC	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Drusen contained cores , basally located regions that were intensely bright when stained for UC or deeply dark when stained for EC ; many were surrounded by concentric lamellae .
	manualset3
250959	5	426593	16	NULL	NULL	0	NULL	EC	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Drusen contained cores , basally located regions that were intensely bright when stained for UC or deeply dark when stained for EC ; many were surrounded by concentric lamellae .
	manualset3
250960	6	426593	16	NULL	NULL	0	NULL	concentric lamellae	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Drusen contained cores , basally located regions that were intensely bright when stained for UC or deeply dark when stained for EC ; many were surrounded by concentric lamellae .
	manualset3
250961	1	426594	16	NULL	NULL	0	NULL	Dual CD45RA , CD45RO positive T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Dual CD45RA , CD45RO positive T cells were found in PB ( up to 74 % ) , SF ( up to 91 % ) and synovium .
	manualset3
250962	2	426594	16	NULL	NULL	0	NULL	PB	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dual CD45RA , CD45RO positive T cells were found in PB ( up to 74 % ) , SF ( up to 91 % ) and synovium .
	manualset3
250963	3	426594	16	NULL	NULL	0	NULL	74 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Dual CD45RA , CD45RO positive T cells were found in PB ( up to 74 % ) , SF ( up to 91 % ) and synovium .
	manualset3
250964	4	426594	16	NULL	NULL	0	NULL	SF	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dual CD45RA , CD45RO positive T cells were found in PB ( up to 74 % ) , SF ( up to 91 % ) and synovium .
	manualset3
250965	5	426594	16	NULL	NULL	0	NULL	91 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Dual CD45RA , CD45RO positive T cells were found in PB ( up to 74 % ) , SF ( up to 91 % ) and synovium .
	manualset3
250966	6	426594	16	NULL	NULL	0	NULL	synovium	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Dual CD45RA , CD45RO positive T cells were found in PB ( up to 74 % ) , SF ( up to 91 % ) and synovium .
	manualset3
250967	1	426595	16	NULL	NULL	0	NULL	Dual malignancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dual malignancy : an interesting concurrent mixed epithelial ovarian tumor with esophageal carcinoma .
	manualset3
250968	2	426595	16	NULL	NULL	0	NULL	concurrent mixed epithelial ovarian tumor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dual malignancy : an interesting concurrent mixed epithelial ovarian tumor with esophageal carcinoma .
	manualset3
250969	3	426595	16	NULL	NULL	0	NULL	esophageal carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Dual malignancy : an interesting concurrent mixed epithelial ovarian tumor with esophageal carcinoma .
	manualset3
250970	1	426596	16	NULL	NULL	0	NULL	DualMesh	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	DualMesh has the potential to become an ideal prosthesis for the bony chest wall as an alternative to conventional polytetrafluoroethylene or polypropylene grafts .
	manualset3
250971	2	426596	16	NULL	NULL	0	NULL	potential	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	DualMesh has the potential to become an ideal prosthesis for the bony chest wall as an alternative to conventional polytetrafluoroethylene or polypropylene grafts .
	manualset3
250972	3	426596	16	NULL	NULL	0	NULL	prosthesis	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	DualMesh has the potential to become an ideal prosthesis for the bony chest wall as an alternative to conventional polytetrafluoroethylene or polypropylene grafts .
	manualset3
250973	4	426596	16	NULL	NULL	0	NULL	bony chest wall	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	DualMesh has the potential to become an ideal prosthesis for the bony chest wall as an alternative to conventional polytetrafluoroethylene or polypropylene grafts .
	manualset3
250974	5	426596	16	NULL	NULL	0	NULL	alternative	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	DualMesh has the potential to become an ideal prosthesis for the bony chest wall as an alternative to conventional polytetrafluoroethylene or polypropylene grafts .
	manualset3
250975	6	426596	16	NULL	NULL	0	NULL	polytetrafluoroethylene grafts	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	DualMesh has the potential to become an ideal prosthesis for the bony chest wall as an alternative to conventional polytetrafluoroethylene or polypropylene grafts .
	manualset3
250976	7	426596	16	NULL	NULL	0	NULL	polypropylene grafts 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	DualMesh has the potential to become an ideal prosthesis for the bony chest wall as an alternative to conventional polytetrafluoroethylene or polypropylene grafts .
	manualset3
250977	1	426597	16	NULL	NULL	0	NULL	Dubin-Johnson pigments	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dubin-Johnson pigments in the hepatocytes decreased in proportion to hepatic regeneration for two months after hepatectomy .
	manualset3
250978	2	426597	16	NULL	NULL	0	NULL	hepatocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Dubin-Johnson pigments in the hepatocytes decreased in proportion to hepatic regeneration for two months after hepatectomy .
	manualset3
250979	3	426597	16	NULL	NULL	0	NULL	proportion	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Dubin-Johnson pigments in the hepatocytes decreased in proportion to hepatic regeneration for two months after hepatectomy .
	manualset3
250980	4	426597	16	NULL	NULL	0	NULL	hepatic regeneration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Dubin-Johnson pigments in the hepatocytes decreased in proportion to hepatic regeneration for two months after hepatectomy .
	manualset3
250981	5	426597	16	NULL	NULL	0	NULL	two months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Dubin-Johnson pigments in the hepatocytes decreased in proportion to hepatic regeneration for two months after hepatectomy .
	manualset3
250982	6	426597	16	NULL	NULL	0	NULL	hepatectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Dubin-Johnson pigments in the hepatocytes decreased in proportion to hepatic regeneration for two months after hepatectomy .
	manualset3
251160	1	426598	16	NULL	NULL	0	NULL	uncertainties	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to inherent uncertainties , a decision is to be made only if the probability of incorrect decision is below a prescribed level .
	manualset3
251165	2	426598	16	NULL	NULL	0	NULL	decision	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to inherent uncertainties , a decision is to be made only if the probability of incorrect decision is below a prescribed level .
	manualset3
251166	3	426598	16	NULL	NULL	0	NULL	probability	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to inherent uncertainties , a decision is to be made only if the probability of incorrect decision is below a prescribed level .
	manualset3
251167	4	426598	16	NULL	NULL	0	NULL	decision	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to inherent uncertainties , a decision is to be made only if the probability of incorrect decision is below a prescribed level .
	manualset3
251168	5	426598	16	NULL	NULL	NULL	NULL	prescribed level	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Due to inherent uncertainties , a decision is to be made only if the probability of incorrect decision is below a prescribed level .
	manualset3
251169	1	426599	16	NULL	NULL	0	NULL	high capacity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to its high capacity and utility in expressing exogenous genes , pEMB0557 will be useful in cloning ( especially silencing genes ) and expressing large DNA fragments ( e.g. , gene clusters ) in B. thuringiensis .
	manualset3
251173	2	426599	16	NULL	NULL	0	NULL	utility	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to its high capacity and utility in expressing exogenous genes , pEMB0557 will be useful in cloning ( especially silencing genes ) and expressing large DNA fragments ( e.g. , gene clusters ) in B. thuringiensis .
	manualset3
251175	3	426599	16	NULL	NULL	0	NULL	exogenous genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to its high capacity and utility in expressing exogenous genes , pEMB0557 will be useful in cloning ( especially silencing genes ) and expressing large DNA fragments ( e.g. , gene clusters ) in B. thuringiensis .
	manualset3
251178	4	426599	16	NULL	NULL	0	NULL	pEMB0557	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to its high capacity and utility in expressing exogenous genes , pEMB0557 will be useful in cloning ( especially silencing genes ) and expressing large DNA fragments ( e.g. , gene clusters ) in B. thuringiensis .
	manualset3
251180	5	426599	16	NULL	NULL	NULL	NULL	cloning	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Due to its high capacity and utility in expressing exogenous genes , pEMB0557 will be useful in cloning ( especially silencing genes ) and expressing large DNA fragments ( e.g. , gene clusters ) in B. thuringiensis .
	manualset3
251185	6	426599	16	NULL	NULL	0	NULL	genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to its high capacity and utility in expressing exogenous genes , pEMB0557 will be useful in cloning ( especially silencing genes ) and expressing large DNA fragments ( e.g. , gene clusters ) in B. thuringiensis .
	manualset3
251186	7	426599	16	NULL	NULL	0	NULL	DNA fragments	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to its high capacity and utility in expressing exogenous genes , pEMB0557 will be useful in cloning ( especially silencing genes ) and expressing large DNA fragments ( e.g. , gene clusters ) in B. thuringiensis .
	manualset3
251188	8	426599	16	NULL	NULL	0	NULL	gene clusters	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to its high capacity and utility in expressing exogenous genes , pEMB0557 will be useful in cloning ( especially silencing genes ) and expressing large DNA fragments ( e.g. , gene clusters ) in B. thuringiensis .
	manualset3
251189	9	426599	16	NULL	NULL	0	NULL	B. thuringiensis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to its high capacity and utility in expressing exogenous genes , pEMB0557 will be useful in cloning ( especially silencing genes ) and expressing large DNA fragments ( e.g. , gene clusters ) in B. thuringiensis .
	manualset3
251206	1	426600	16	NULL	NULL	0	NULL	binding activity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to lack of appropriate binding activity of the material obtained , we decided to use a kit which provides solubilized porcine membrane-receptors to TSH instead of human membranes , as well as calibrators that have been standardized in a receptor assay against MRC LATS std B. With these reactives we have measured TRAb in sera from 7 normal controls ( C ) , 54 thyrotoxic patients ( 43 diffuse goiters ( BDH ) , 8 multinodular goiters ( BHM ) and 3 Subacute Thyroiditis ( TSA ) ) , 3 patients with Hashimoto 's Thyroiditis ( TH ) and in 6 non-hyperthyroid Graves ophthalmopathy patients .
	manualset3
251207	2	426600	16	NULL	NULL	NULL	NULL	material	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Due to lack of appropriate binding activity of the material obtained , we decided to use a kit which provides solubilized porcine membrane-receptors to TSH instead of human membranes , as well as calibrators that have been standardized in a receptor assay against MRC LATS std B. With these reactives we have measured TRAb in sera from 7 normal controls ( C ) , 54 thyrotoxic patients ( 43 diffuse goiters ( BDH ) , 8 multinodular goiters ( BHM ) and 3 Subacute Thyroiditis ( TSA ) ) , 3 patients with Hashimoto 's Thyroiditis ( TH ) and in 6 non-hyperthyroid Graves ophthalmopathy patients .
	manualset3
251208	3	426600	16	NULL	NULL	NULL	NULL	kit	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Due to lack of appropriate binding activity of the material obtained , we decided to use a kit which provides solubilized porcine membrane-receptors to TSH instead of human membranes , as well as calibrators that have been standardized in a receptor assay against MRC LATS std B. With these reactives we have measured TRAb in sera from 7 normal controls ( C ) , 54 thyrotoxic patients ( 43 diffuse goiters ( BDH ) , 8 multinodular goiters ( BHM ) and 3 Subacute Thyroiditis ( TSA ) ) , 3 patients with Hashimoto 's Thyroiditis ( TH ) and in 6 non-hyperthyroid Graves ophthalmopathy patients .
	manualset3
251209	4	426600	16	NULL	NULL	0	NULL	porcine membrane-receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to lack of appropriate binding activity of the material obtained , we decided to use a kit which provides solubilized porcine membrane-receptors to TSH instead of human membranes , as well as calibrators that have been standardized in a receptor assay against MRC LATS std B. With these reactives we have measured TRAb in sera from 7 normal controls ( C ) , 54 thyrotoxic patients ( 43 diffuse goiters ( BDH ) , 8 multinodular goiters ( BHM ) and 3 Subacute Thyroiditis ( TSA ) ) , 3 patients with Hashimoto 's Thyroiditis ( TH ) and in 6 non-hyperthyroid Graves ophthalmopathy patients .
	manualset3
251210	5	426600	16	NULL	NULL	0	NULL	TSH	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to lack of appropriate binding activity of the material obtained , we decided to use a kit which provides solubilized porcine membrane-receptors to TSH instead of human membranes , as well as calibrators that have been standardized in a receptor assay against MRC LATS std B. With these reactives we have measured TRAb in sera from 7 normal controls ( C ) , 54 thyrotoxic patients ( 43 diffuse goiters ( BDH ) , 8 multinodular goiters ( BHM ) and 3 Subacute Thyroiditis ( TSA ) ) , 3 patients with Hashimoto 's Thyroiditis ( TH ) and in 6 non-hyperthyroid Graves ophthalmopathy patients .
	manualset3
251211	6	426600	16	NULL	NULL	0	NULL	human membranes	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to lack of appropriate binding activity of the material obtained , we decided to use a kit which provides solubilized porcine membrane-receptors to TSH instead of human membranes , as well as calibrators that have been standardized in a receptor assay against MRC LATS std B. With these reactives we have measured TRAb in sera from 7 normal controls ( C ) , 54 thyrotoxic patients ( 43 diffuse goiters ( BDH ) , 8 multinodular goiters ( BHM ) and 3 Subacute Thyroiditis ( TSA ) ) , 3 patients with Hashimoto 's Thyroiditis ( TH ) and in 6 non-hyperthyroid Graves ophthalmopathy patients .
	manualset3
251212	7	426600	16	NULL	NULL	0	NULL	calibrators	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to lack of appropriate binding activity of the material obtained , we decided to use a kit which provides solubilized porcine membrane-receptors to TSH instead of human membranes , as well as calibrators that have been standardized in a receptor assay against MRC LATS std B. With these reactives we have measured TRAb in sera from 7 normal controls ( C ) , 54 thyrotoxic patients ( 43 diffuse goiters ( BDH ) , 8 multinodular goiters ( BHM ) and 3 Subacute Thyroiditis ( TSA ) ) , 3 patients with Hashimoto 's Thyroiditis ( TH ) and in 6 non-hyperthyroid Graves ophthalmopathy patients .
	manualset3
251213	8	426600	16	NULL	NULL	0	NULL	receptor assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to lack of appropriate binding activity of the material obtained , we decided to use a kit which provides solubilized porcine membrane-receptors to TSH instead of human membranes , as well as calibrators that have been standardized in a receptor assay against MRC LATS std B. With these reactives we have measured TRAb in sera from 7 normal controls ( C ) , 54 thyrotoxic patients ( 43 diffuse goiters ( BDH ) , 8 multinodular goiters ( BHM ) and 3 Subacute Thyroiditis ( TSA ) ) , 3 patients with Hashimoto 's Thyroiditis ( TH ) and in 6 non-hyperthyroid Graves ophthalmopathy patients .
	manualset3
251214	9	426600	16	NULL	NULL	0	NULL	MRC LATS std B	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to lack of appropriate binding activity of the material obtained , we decided to use a kit which provides solubilized porcine membrane-receptors to TSH instead of human membranes , as well as calibrators that have been standardized in a receptor assay against MRC LATS std B. With these reactives we have measured TRAb in sera from 7 normal controls ( C ) , 54 thyrotoxic patients ( 43 diffuse goiters ( BDH ) , 8 multinodular goiters ( BHM ) and 3 Subacute Thyroiditis ( TSA ) ) , 3 patients with Hashimoto 's Thyroiditis ( TH ) and in 6 non-hyperthyroid Graves ophthalmopathy patients .
	manualset3
251215	10	426600	16	NULL	NULL	0	NULL	reactives	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to lack of appropriate binding activity of the material obtained , we decided to use a kit which provides solubilized porcine membrane-receptors to TSH instead of human membranes , as well as calibrators that have been standardized in a receptor assay against MRC LATS std B. With these reactives we have measured TRAb in sera from 7 normal controls ( C ) , 54 thyrotoxic patients ( 43 diffuse goiters ( BDH ) , 8 multinodular goiters ( BHM ) and 3 Subacute Thyroiditis ( TSA ) ) , 3 patients with Hashimoto 's Thyroiditis ( TH ) and in 6 non-hyperthyroid Graves ophthalmopathy patients .
	manualset3
251238	11	426600	16	NULL	NULL	0	NULL	sera	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to lack of appropriate binding activity of the material obtained , we decided to use a kit which provides solubilized porcine membrane-receptors to TSH instead of human membranes , as well as calibrators that have been standardized in a receptor assay against MRC LATS std B. With these reactives we have measured TRAb in sera from 7 normal controls ( C ) , 54 thyrotoxic patients ( 43 diffuse goiters ( BDH ) , 8 multinodular goiters ( BHM ) and 3 Subacute Thyroiditis ( TSA ) ) , 3 patients with Hashimoto 's Thyroiditis ( TH ) and in 6 non-hyperthyroid Graves ophthalmopathy patients .
	manualset3
251241	12	426600	16	NULL	NULL	0	NULL	7 normal controls ( C )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to lack of appropriate binding activity of the material obtained , we decided to use a kit which provides solubilized porcine membrane-receptors to TSH instead of human membranes , as well as calibrators that have been standardized in a receptor assay against MRC LATS std B. With these reactives we have measured TRAb in sera from 7 normal controls ( C ) , 54 thyrotoxic patients ( 43 diffuse goiters ( BDH ) , 8 multinodular goiters ( BHM ) and 3 Subacute Thyroiditis ( TSA ) ) , 3 patients with Hashimoto 's Thyroiditis ( TH ) and in 6 non-hyperthyroid Graves ophthalmopathy patients .
	manualset3
251243	13	426600	16	NULL	NULL	0	NULL	54 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to lack of appropriate binding activity of the material obtained , we decided to use a kit which provides solubilized porcine membrane-receptors to TSH instead of human membranes , as well as calibrators that have been standardized in a receptor assay against MRC LATS std B. With these reactives we have measured TRAb in sera from 7 normal controls ( C ) , 54 thyrotoxic patients ( 43 diffuse goiters ( BDH ) , 8 multinodular goiters ( BHM ) and 3 Subacute Thyroiditis ( TSA ) ) , 3 patients with Hashimoto 's Thyroiditis ( TH ) and in 6 non-hyperthyroid Graves ophthalmopathy patients .
	manualset3
251244	14	426600	16	NULL	NULL	0	NULL	thyrotoxic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to lack of appropriate binding activity of the material obtained , we decided to use a kit which provides solubilized porcine membrane-receptors to TSH instead of human membranes , as well as calibrators that have been standardized in a receptor assay against MRC LATS std B. With these reactives we have measured TRAb in sera from 7 normal controls ( C ) , 54 thyrotoxic patients ( 43 diffuse goiters ( BDH ) , 8 multinodular goiters ( BHM ) and 3 Subacute Thyroiditis ( TSA ) ) , 3 patients with Hashimoto 's Thyroiditis ( TH ) and in 6 non-hyperthyroid Graves ophthalmopathy patients .
	manualset3
251249	15	426600	16	NULL	NULL	0	NULL	43	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to lack of appropriate binding activity of the material obtained , we decided to use a kit which provides solubilized porcine membrane-receptors to TSH instead of human membranes , as well as calibrators that have been standardized in a receptor assay against MRC LATS std B. With these reactives we have measured TRAb in sera from 7 normal controls ( C ) , 54 thyrotoxic patients ( 43 diffuse goiters ( BDH ) , 8 multinodular goiters ( BHM ) and 3 Subacute Thyroiditis ( TSA ) ) , 3 patients with Hashimoto 's Thyroiditis ( TH ) and in 6 non-hyperthyroid Graves ophthalmopathy patients .
	manualset3
251250	16	426600	16	NULL	NULL	0	NULL	diffuse goiters ( BDH )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to lack of appropriate binding activity of the material obtained , we decided to use a kit which provides solubilized porcine membrane-receptors to TSH instead of human membranes , as well as calibrators that have been standardized in a receptor assay against MRC LATS std B. With these reactives we have measured TRAb in sera from 7 normal controls ( C ) , 54 thyrotoxic patients ( 43 diffuse goiters ( BDH ) , 8 multinodular goiters ( BHM ) and 3 Subacute Thyroiditis ( TSA ) ) , 3 patients with Hashimoto 's Thyroiditis ( TH ) and in 6 non-hyperthyroid Graves ophthalmopathy patients .
	manualset3
251251	17	426600	16	NULL	NULL	0	NULL	8	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to lack of appropriate binding activity of the material obtained , we decided to use a kit which provides solubilized porcine membrane-receptors to TSH instead of human membranes , as well as calibrators that have been standardized in a receptor assay against MRC LATS std B. With these reactives we have measured TRAb in sera from 7 normal controls ( C ) , 54 thyrotoxic patients ( 43 diffuse goiters ( BDH ) , 8 multinodular goiters ( BHM ) and 3 Subacute Thyroiditis ( TSA ) ) , 3 patients with Hashimoto 's Thyroiditis ( TH ) and in 6 non-hyperthyroid Graves ophthalmopathy patients .
	manualset3
251252	18	426600	16	NULL	NULL	0	NULL	multinodular goiters ( BHM )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to lack of appropriate binding activity of the material obtained , we decided to use a kit which provides solubilized porcine membrane-receptors to TSH instead of human membranes , as well as calibrators that have been standardized in a receptor assay against MRC LATS std B. With these reactives we have measured TRAb in sera from 7 normal controls ( C ) , 54 thyrotoxic patients ( 43 diffuse goiters ( BDH ) , 8 multinodular goiters ( BHM ) and 3 Subacute Thyroiditis ( TSA ) ) , 3 patients with Hashimoto 's Thyroiditis ( TH ) and in 6 non-hyperthyroid Graves ophthalmopathy patients .
	manualset3
251253	19	426600	16	NULL	NULL	0	NULL	3	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to lack of appropriate binding activity of the material obtained , we decided to use a kit which provides solubilized porcine membrane-receptors to TSH instead of human membranes , as well as calibrators that have been standardized in a receptor assay against MRC LATS std B. With these reactives we have measured TRAb in sera from 7 normal controls ( C ) , 54 thyrotoxic patients ( 43 diffuse goiters ( BDH ) , 8 multinodular goiters ( BHM ) and 3 Subacute Thyroiditis ( TSA ) ) , 3 patients with Hashimoto 's Thyroiditis ( TH ) and in 6 non-hyperthyroid Graves ophthalmopathy patients .
	manualset3
251254	20	426600	16	NULL	NULL	0	NULL	Subacute Thyroiditis ( TSA )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to lack of appropriate binding activity of the material obtained , we decided to use a kit which provides solubilized porcine membrane-receptors to TSH instead of human membranes , as well as calibrators that have been standardized in a receptor assay against MRC LATS std B. With these reactives we have measured TRAb in sera from 7 normal controls ( C ) , 54 thyrotoxic patients ( 43 diffuse goiters ( BDH ) , 8 multinodular goiters ( BHM ) and 3 Subacute Thyroiditis ( TSA ) ) , 3 patients with Hashimoto 's Thyroiditis ( TH ) and in 6 non-hyperthyroid Graves ophthalmopathy patients .
	manualset3
251255	21	426600	16	NULL	NULL	0	NULL	3 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to lack of appropriate binding activity of the material obtained , we decided to use a kit which provides solubilized porcine membrane-receptors to TSH instead of human membranes , as well as calibrators that have been standardized in a receptor assay against MRC LATS std B. With these reactives we have measured TRAb in sera from 7 normal controls ( C ) , 54 thyrotoxic patients ( 43 diffuse goiters ( BDH ) , 8 multinodular goiters ( BHM ) and 3 Subacute Thyroiditis ( TSA ) ) , 3 patients with Hashimoto 's Thyroiditis ( TH ) and in 6 non-hyperthyroid Graves ophthalmopathy patients .
	manualset3
251256	22	426600	16	NULL	NULL	0	NULL	6	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to lack of appropriate binding activity of the material obtained , we decided to use a kit which provides solubilized porcine membrane-receptors to TSH instead of human membranes , as well as calibrators that have been standardized in a receptor assay against MRC LATS std B. With these reactives we have measured TRAb in sera from 7 normal controls ( C ) , 54 thyrotoxic patients ( 43 diffuse goiters ( BDH ) , 8 multinodular goiters ( BHM ) and 3 Subacute Thyroiditis ( TSA ) ) , 3 patients with Hashimoto 's Thyroiditis ( TH ) and in 6 non-hyperthyroid Graves ophthalmopathy patients .
	manualset3
251257	23	426600	16	NULL	NULL	0	NULL	non-hyperthyroid Graves ophthalmopathy	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to lack of appropriate binding activity of the material obtained , we decided to use a kit which provides solubilized porcine membrane-receptors to TSH instead of human membranes , as well as calibrators that have been standardized in a receptor assay against MRC LATS std B. With these reactives we have measured TRAb in sera from 7 normal controls ( C ) , 54 thyrotoxic patients ( 43 diffuse goiters ( BDH ) , 8 multinodular goiters ( BHM ) and 3 Subacute Thyroiditis ( TSA ) ) , 3 patients with Hashimoto 's Thyroiditis ( TH ) and in 6 non-hyperthyroid Graves ophthalmopathy patients .
	manualset3
251259	24	426600	16	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to lack of appropriate binding activity of the material obtained , we decided to use a kit which provides solubilized porcine membrane-receptors to TSH instead of human membranes , as well as calibrators that have been standardized in a receptor assay against MRC LATS std B. With these reactives we have measured TRAb in sera from 7 normal controls ( C ) , 54 thyrotoxic patients ( 43 diffuse goiters ( BDH ) , 8 multinodular goiters ( BHM ) and 3 Subacute Thyroiditis ( TSA ) ) , 3 patients with Hashimoto 's Thyroiditis ( TH ) and in 6 non-hyperthyroid Graves ophthalmopathy patients .
	manualset3
251263	1	426601	16	NULL	NULL	NULL	NULL	microbiological diagnosis	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Due to rapid microbiological diagnosis-direct microscopical examination of muscle biopsies revealed numerous grampositive rods - , immediately performed amputation of the leg and antibiotic treatment with penicillin and metronidazole the patient survived .
	manualset3
251264	2	426601	16	NULL	NULL	0	NULL	muscle biopsies	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to rapid microbiological diagnosis-direct microscopical examination of muscle biopsies revealed numerous grampositive rods - , immediately performed amputation of the leg and antibiotic treatment with penicillin and metronidazole the patient survived .
	manualset3
251265	3	426601	16	NULL	NULL	0	NULL	grampositive rods	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to rapid microbiological diagnosis-direct microscopical examination of muscle biopsies revealed numerous grampositive rods - , immediately performed amputation of the leg and antibiotic treatment with penicillin and metronidazole the patient survived .
	manualset3
251266	4	426601	16	NULL	NULL	0	NULL	amputation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to rapid microbiological diagnosis-direct microscopical examination of muscle biopsies revealed numerous grampositive rods - , immediately performed amputation of the leg and antibiotic treatment with penicillin and metronidazole the patient survived .
	manualset3
251268	5	426601	16	NULL	NULL	0	NULL	leg	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to rapid microbiological diagnosis-direct microscopical examination of muscle biopsies revealed numerous grampositive rods - , immediately performed amputation of the leg and antibiotic treatment with penicillin and metronidazole the patient survived .
	manualset3
251270	6	426601	16	NULL	NULL	0	NULL	antibiotic treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to rapid microbiological diagnosis-direct microscopical examination of muscle biopsies revealed numerous grampositive rods - , immediately performed amputation of the leg and antibiotic treatment with penicillin and metronidazole the patient survived .
	manualset3
251272	7	426601	16	NULL	NULL	0	NULL	penicillin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to rapid microbiological diagnosis-direct microscopical examination of muscle biopsies revealed numerous grampositive rods - , immediately performed amputation of the leg and antibiotic treatment with penicillin and metronidazole the patient survived .
	manualset3
251273	8	426601	16	NULL	NULL	0	NULL	metronidazole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to rapid microbiological diagnosis-direct microscopical examination of muscle biopsies revealed numerous grampositive rods - , immediately performed amputation of the leg and antibiotic treatment with penicillin and metronidazole the patient survived .
	manualset3
251274	9	426601	16	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to rapid microbiological diagnosis-direct microscopical examination of muscle biopsies revealed numerous grampositive rods - , immediately performed amputation of the leg and antibiotic treatment with penicillin and metronidazole the patient survived .
	manualset3
251284	10	426601	16	NULL	NULL	0	NULL	direct microscopical examination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to rapid microbiological diagnosis-direct microscopical examination of muscle biopsies revealed numerous grampositive rods - , immediately performed amputation of the leg and antibiotic treatment with penicillin and metronidazole the patient survived .
	manualset3
251286	1	426602	16	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to the addition of NH ( 4 ) NO ( 3 ) fertilizer and subsequent nitrification of ammonia to nitrate , soil pH decreased from 4.7 to 3.5 and from 5.5 to 4 , respectively .
	manualset3
251288	2	426602	16	NULL	NULL	0	NULL	NH ( 4 ) NO ( 3 ) fertilizer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to the addition of NH ( 4 ) NO ( 3 ) fertilizer and subsequent nitrification of ammonia to nitrate , soil pH decreased from 4.7 to 3.5 and from 5.5 to 4 , respectively .
	manualset3
251290	3	426602	16	NULL	NULL	0	NULL	nitrification	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to the addition of NH ( 4 ) NO ( 3 ) fertilizer and subsequent nitrification of ammonia to nitrate , soil pH decreased from 4.7 to 3.5 and from 5.5 to 4 , respectively .
	manualset3
251291	4	426602	16	NULL	NULL	0	NULL	ammonia	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to the addition of NH ( 4 ) NO ( 3 ) fertilizer and subsequent nitrification of ammonia to nitrate , soil pH decreased from 4.7 to 3.5 and from 5.5 to 4 , respectively .
	manualset3
251292	5	426602	16	NULL	NULL	0	NULL	nitrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to the addition of NH ( 4 ) NO ( 3 ) fertilizer and subsequent nitrification of ammonia to nitrate , soil pH decreased from 4.7 to 3.5 and from 5.5 to 4 , respectively .
	manualset3
251294	6	426602	16	NULL	NULL	NULL	NULL	soil pH	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Due to the addition of NH ( 4 ) NO ( 3 ) fertilizer and subsequent nitrification of ammonia to nitrate , soil pH decreased from 4.7 to 3.5 and from 5.5 to 4 , respectively .
	manualset3
251296	7	426602	16	NULL	NULL	0	NULL	4.7 to 3.5	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to the addition of NH ( 4 ) NO ( 3 ) fertilizer and subsequent nitrification of ammonia to nitrate , soil pH decreased from 4.7 to 3.5 and from 5.5 to 4 , respectively .
	manualset3
251298	8	426602	16	NULL	NULL	0	NULL	5.5 to 4	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to the addition of NH ( 4 ) NO ( 3 ) fertilizer and subsequent nitrification of ammonia to nitrate , soil pH decreased from 4.7 to 3.5 and from 5.5 to 4 , respectively .
	manualset3
251304	1	426603	16	NULL	NULL	0	NULL	absence of clinical symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to the complete absence of clinical symptoms or a fistula connecting the prosthesis and the aneurysm or progress in size of the aneurysm during the follow-up period the third patient was treated conservatively .
	manualset3
251305	2	426603	16	NULL	NULL	0	NULL	fistula	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to the complete absence of clinical symptoms or a fistula connecting the prosthesis and the aneurysm or progress in size of the aneurysm during the follow-up period the third patient was treated conservatively .
	manualset3
251307	3	426603	16	NULL	NULL	0	NULL	prosthesis	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to the complete absence of clinical symptoms or a fistula connecting the prosthesis and the aneurysm or progress in size of the aneurysm during the follow-up period the third patient was treated conservatively .
	manualset3
251308	4	426603	16	NULL	NULL	0	NULL	aneurysm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to the complete absence of clinical symptoms or a fistula connecting the prosthesis and the aneurysm or progress in size of the aneurysm during the follow-up period the third patient was treated conservatively .
	manualset3
251318	5	426603	16	NULL	NULL	NULL	NULL	size	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Due to the complete absence of clinical symptoms or a fistula connecting the prosthesis and the aneurysm or progress in size of the aneurysm during the follow-up period the third patient was treated conservatively .
	manualset3
251320	6	426603	16	NULL	NULL	NULL	NULL	aneurysm	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Due to the complete absence of clinical symptoms or a fistula connecting the prosthesis and the aneurysm or progress in size of the aneurysm during the follow-up period the third patient was treated conservatively .
	manualset3
251322	7	426603	16	NULL	NULL	NULL	NULL	follow-up period	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Due to the complete absence of clinical symptoms or a fistula connecting the prosthesis and the aneurysm or progress in size of the aneurysm during the follow-up period the third patient was treated conservatively .
	manualset3
251324	8	426603	16	NULL	NULL	NULL	NULL	third patient	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Due to the complete absence of clinical symptoms or a fistula connecting the prosthesis and the aneurysm or progress in size of the aneurysm during the follow-up period the third patient was treated conservatively .
	manualset3
251344	1	426604	16	NULL	NULL	0	NULL	problem	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the problem of the preservation of ear cartilage in ophthalmology ) .
	manualset3
251346	2	426604	16	NULL	NULL	0	NULL	preservation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the problem of the preservation of ear cartilage in ophthalmology ) .
	manualset3
251351	3	426604	16	NULL	NULL	0	NULL	ear cartilage	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the problem of the preservation of ear cartilage in ophthalmology ) .
	manualset3
251355	4	426604	16	NULL	NULL	0	NULL	ophthalmology	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the problem of the preservation of ear cartilage in ophthalmology ) .
	manualset3
251618	1	426605	16	NULL	NULL	0	NULL	lack	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to the lack of endogenous enzymes responsible for ONOO - scavenging activity , finding a specific ONOO - scavenger is of considerable importance .
	manualset3
251619	2	426605	16	NULL	NULL	0	NULL	enzymes	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to the lack of endogenous enzymes responsible for ONOO - scavenging activity , finding a specific ONOO - scavenger is of considerable importance .
	manualset3
251620	3	426605	16	NULL	NULL	0	NULL	ONOO - scavenging activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to the lack of endogenous enzymes responsible for ONOO - scavenging activity , finding a specific ONOO - scavenger is of considerable importance .
	manualset3
251621	4	426605	16	NULL	NULL	0	NULL	ONOO - scavenger	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to the lack of endogenous enzymes responsible for ONOO - scavenging activity , finding a specific ONOO - scavenger is of considerable importance .
	manualset3
251622	1	426606	16	NULL	NULL	0	NULL	location	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to the location around the pancreatoduodenal region or the strong possibility of injury to a major vessel , 39 contained retroperitoneal hematomas and were explored .
	manualset3
251623	2	426606	16	NULL	NULL	0	NULL	pancreatoduodenal region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to the location around the pancreatoduodenal region or the strong possibility of injury to a major vessel , 39 contained retroperitoneal hematomas and were explored .
	manualset3
251624	3	426606	16	NULL	NULL	0	NULL	possibility	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to the location around the pancreatoduodenal region or the strong possibility of injury to a major vessel , 39 contained retroperitoneal hematomas and were explored .
	manualset3
251625	4	426606	16	NULL	NULL	0	NULL	injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to the location around the pancreatoduodenal region or the strong possibility of injury to a major vessel , 39 contained retroperitoneal hematomas and were explored .
	manualset3
251626	5	426606	16	NULL	NULL	0	NULL	major vessel	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to the location around the pancreatoduodenal region or the strong possibility of injury to a major vessel , 39 contained retroperitoneal hematomas and were explored .
	manualset3
251627	6	426606	16	NULL	NULL	0	NULL	39	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to the location around the pancreatoduodenal region or the strong possibility of injury to a major vessel , 39 contained retroperitoneal hematomas and were explored .
	manualset3
251628	7	426606	16	NULL	NULL	0	NULL	retroperitoneal hematomas	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to the location around the pancreatoduodenal region or the strong possibility of injury to a major vessel , 39 contained retroperitoneal hematomas and were explored .
	manualset3
251629	1	426607	16	NULL	NULL	0	NULL	nonmonotonic growth pattern	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to the nonmonotonic growth pattern of the correlation-based similarity measures , partial computation elimination techniques have been traditionally considered inapplicable to speed up these measures .
	manualset3
251630	2	426607	16	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to the nonmonotonic growth pattern of the correlation-based similarity measures , partial computation elimination techniques have been traditionally considered inapplicable to speed up these measures .
	manualset3
251631	3	426607	16	NULL	NULL	0	NULL	similarity measures	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to the nonmonotonic growth pattern of the correlation-based similarity measures , partial computation elimination techniques have been traditionally considered inapplicable to speed up these measures .
	manualset3
251632	4	426607	16	NULL	NULL	0	NULL	partial computation elimination techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to the nonmonotonic growth pattern of the correlation-based similarity measures , partial computation elimination techniques have been traditionally considered inapplicable to speed up these measures .
	manualset3
251633	5	426607	16	NULL	NULL	0	NULL	measures	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to the nonmonotonic growth pattern of the correlation-based similarity measures , partial computation elimination techniques have been traditionally considered inapplicable to speed up these measures .
	manualset3
251634	1	426608	16	NULL	NULL	0	NULL	rarity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to the rarity of JDM clinical trials will have to be performed on an international basis .
	manualset3
251635	2	426608	16	NULL	NULL	0	NULL	JDM clinical trials	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Due to the rarity of JDM clinical trials will have to be performed on an international basis .
	manualset3
251636	3	426608	16	NULL	NULL	NULL	NULL	basis	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Due to the rarity of JDM clinical trials will have to be performed on an international basis .
	manualset3
251637	1	426609	16	NULL	NULL	NULL	NULL	lung	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dueling in the lung : how Cryptococcus spores race the host for survival .
	manualset3
251638	2	426609	16	NULL	NULL	0	NULL	Cryptococcus spores	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Dueling in the lung : how Cryptococcus spores race the host for survival .
	manualset3
251639	3	426609	16	NULL	NULL	0	NULL	host	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Dueling in the lung : how Cryptococcus spores race the host for survival .
	manualset3
251640	4	426609	16	NULL	NULL	0	NULL	survival	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dueling in the lung : how Cryptococcus spores race the host for survival .
	manualset3
251641	1	426610	16	NULL	NULL	0	NULL	Dumbbell synovial sarcoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Dumbbell synovial sarcoma of the thoracolumbar spine : a case report .
	manualset3
251642	2	426610	16	NULL	NULL	0	NULL	thoracolumbar spine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Dumbbell synovial sarcoma of the thoracolumbar spine : a case report .
	manualset3
251643	3	426610	16	NULL	NULL	0	NULL	case report	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Dumbbell synovial sarcoma of the thoracolumbar spine : a case report .
	manualset3
251644	1	426611	16	NULL	NULL	0	NULL	Duodenal adenocarcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Duodenal adenocarcinoma : clinicopathologic analysis and implications for treatment .
	manualset3
251645	2	426611	16	NULL	NULL	0	NULL	clinicopathologic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Duodenal adenocarcinoma : clinicopathologic analysis and implications for treatment .
	manualset3
251646	3	426611	16	NULL	NULL	0	NULL	implications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Duodenal adenocarcinoma : clinicopathologic analysis and implications for treatment .
	manualset3
251647	4	426611	16	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Duodenal adenocarcinoma : clinicopathologic analysis and implications for treatment .
	manualset3
251648	1	426612	16	NULL	NULL	0	NULL	problem	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the problem of the status of portal blood flow in patients with opisthorchosis ) .
	manualset3
251649	2	426612	16	NULL	NULL	0	NULL	status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the problem of the status of portal blood flow in patients with opisthorchosis ) .
	manualset3
251650	3	426612	16	NULL	NULL	0	NULL	portal blood flow	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the problem of the status of portal blood flow in patients with opisthorchosis ) .
	manualset3
251651	4	426612	16	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the problem of the status of portal blood flow in patients with opisthorchosis ) .
	manualset3
251652	5	426612	16	NULL	NULL	0	NULL	opisthorchosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the problem of the status of portal blood flow in patients with opisthorchosis ) .
	manualset3
251653	1	426613	16	NULL	NULL	0	NULL	Duodenal diverticulum	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Duodenal diverticulum is a common anatomic abnormality .
	manualset3
251654	2	426613	16	NULL	NULL	0	NULL	anatomic abnormality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Duodenal diverticulum is a common anatomic abnormality .
	manualset3
251655	1	426614	16	NULL	NULL	0	NULL	Duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Duration and predictors of CD4 T-cell gains in patients who continue combination therapy despite detectable plasma viremia .
	manualset3
251656	2	426614	16	NULL	NULL	0	NULL	predictors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Duration and predictors of CD4 T-cell gains in patients who continue combination therapy despite detectable plasma viremia .
	manualset3
251657	3	426614	16	NULL	NULL	0	NULL	CD4 T-cell gains	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Duration and predictors of CD4 T-cell gains in patients who continue combination therapy despite detectable plasma viremia .
	manualset3
251658	4	426614	16	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Duration and predictors of CD4 T-cell gains in patients who continue combination therapy despite detectable plasma viremia .
	manualset3
251659	5	426614	16	NULL	NULL	0	NULL	combination therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Duration and predictors of CD4 T-cell gains in patients who continue combination therapy despite detectable plasma viremia .
	manualset3
251660	6	426614	16	NULL	NULL	0	NULL	plasma viremia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Duration and predictors of CD4 T-cell gains in patients who continue combination therapy despite detectable plasma viremia .
	manualset3
251661	1	426615	16	NULL	NULL	0	NULL	1 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	During 1 min of reperfusion following regional ischemia the level of citrate increased 460 % , to approximately 600 nmol g-1 wet weight .
	manualset3
251662	2	426615	16	NULL	NULL	0	NULL	reperfusion	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	During 1 min of reperfusion following regional ischemia the level of citrate increased 460 % , to approximately 600 nmol g-1 wet weight .
	manualset3
251663	3	426615	16	NULL	NULL	0	NULL	regional ischemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	During 1 min of reperfusion following regional ischemia the level of citrate increased 460 % , to approximately 600 nmol g-1 wet weight .
	manualset3
251664	4	426615	16	NULL	NULL	0	NULL	level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	During 1 min of reperfusion following regional ischemia the level of citrate increased 460 % , to approximately 600 nmol g-1 wet weight .
	manualset3
251665	5	426615	16	NULL	NULL	0	NULL	citrate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	During 1 min of reperfusion following regional ischemia the level of citrate increased 460 % , to approximately 600 nmol g-1 wet weight .
	manualset3
251666	6	426615	16	NULL	NULL	0	NULL	460 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During 1 min of reperfusion following regional ischemia the level of citrate increased 460 % , to approximately 600 nmol g-1 wet weight .
	manualset3
251667	7	426615	16	NULL	NULL	0	NULL	600 nmol g-1	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During 1 min of reperfusion following regional ischemia the level of citrate increased 460 % , to approximately 600 nmol g-1 wet weight .
	manualset3
251668	8	426615	16	NULL	NULL	0	NULL	wet weight	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During 1 min of reperfusion following regional ischemia the level of citrate increased 460 % , to approximately 600 nmol g-1 wet weight .
	manualset3
251669	1	426616	16	NULL	NULL	0	NULL	10 min	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	During 10 min exposure in a 60 x 75 x 22 cm open field ( OF ) we found higher rates of infrared beam crossing on pd 12-14 , more rearing on pd 12 , 16 and 32 and less immobility of MSG rats .
	manualset3
251670	2	426616	16	NULL	NULL	0	NULL	exposure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	During 10 min exposure in a 60 x 75 x 22 cm open field ( OF ) we found higher rates of infrared beam crossing on pd 12-14 , more rearing on pd 12 , 16 and 32 and less immobility of MSG rats .
	manualset3
251671	3	426616	16	NULL	NULL	0	NULL	60 x 75 x 22 cm open field ( OF )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During 10 min exposure in a 60 x 75 x 22 cm open field ( OF ) we found higher rates of infrared beam crossing on pd 12-14 , more rearing on pd 12 , 16 and 32 and less immobility of MSG rats .
	manualset3
251672	4	426616	16	NULL	NULL	NULL	NULL	rates of infrared beam crossing	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During 10 min exposure in a 60 x 75 x 22 cm open field ( OF ) we found higher rates of infrared beam crossing on pd 12-14 , more rearing on pd 12 , 16 and 32 and less immobility of MSG rats .
	manualset3
251673	5	426616	16	NULL	NULL	NULL	NULL	pd 12-14	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During 10 min exposure in a 60 x 75 x 22 cm open field ( OF ) we found higher rates of infrared beam crossing on pd 12-14 , more rearing on pd 12 , 16 and 32 and less immobility of MSG rats .
	manualset3
251674	6	426616	16	NULL	NULL	0	NULL	rearing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	During 10 min exposure in a 60 x 75 x 22 cm open field ( OF ) we found higher rates of infrared beam crossing on pd 12-14 , more rearing on pd 12 , 16 and 32 and less immobility of MSG rats .
	manualset3
251675	7	426616	16	NULL	NULL	0	NULL	pd 12	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	During 10 min exposure in a 60 x 75 x 22 cm open field ( OF ) we found higher rates of infrared beam crossing on pd 12-14 , more rearing on pd 12 , 16 and 32 and less immobility of MSG rats .
	manualset3
251676	8	426616	16	NULL	NULL	0	NULL	pd 16	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	During 10 min exposure in a 60 x 75 x 22 cm open field ( OF ) we found higher rates of infrared beam crossing on pd 12-14 , more rearing on pd 12 , 16 and 32 and less immobility of MSG rats .
	manualset3
251677	9	426616	16	NULL	NULL	0	NULL	pd 32	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	During 10 min exposure in a 60 x 75 x 22 cm open field ( OF ) we found higher rates of infrared beam crossing on pd 12-14 , more rearing on pd 12 , 16 and 32 and less immobility of MSG rats .
	manualset3
251678	10	426616	16	NULL	NULL	0	NULL	immobility	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	During 10 min exposure in a 60 x 75 x 22 cm open field ( OF ) we found higher rates of infrared beam crossing on pd 12-14 , more rearing on pd 12 , 16 and 32 and less immobility of MSG rats .
	manualset3
251679	11	426616	16	NULL	NULL	0	NULL	MSG rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	During 10 min exposure in a 60 x 75 x 22 cm open field ( OF ) we found higher rates of infrared beam crossing on pd 12-14 , more rearing on pd 12 , 16 and 32 and less immobility of MSG rats .
	manualset3
251680	1	426617	16	NULL	NULL	0	NULL	16 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	During 16 years of follow-up of overweight subjects , 188 men and 44 women had CHD events , indicating an age-adjusted rate that was not much different from the slim subjects .
	manualset3
251681	2	426617	16	NULL	NULL	0	NULL	follow-up	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	During 16 years of follow-up of overweight subjects , 188 men and 44 women had CHD events , indicating an age-adjusted rate that was not much different from the slim subjects .
	manualset3
251682	3	426617	16	NULL	NULL	0	NULL	overweight subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	During 16 years of follow-up of overweight subjects , 188 men and 44 women had CHD events , indicating an age-adjusted rate that was not much different from the slim subjects .
	manualset3
251683	4	426617	16	NULL	NULL	0	NULL	188 men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	During 16 years of follow-up of overweight subjects , 188 men and 44 women had CHD events , indicating an age-adjusted rate that was not much different from the slim subjects .
	manualset3
251684	5	426617	16	NULL	NULL	0	NULL	44 women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	During 16 years of follow-up of overweight subjects , 188 men and 44 women had CHD events , indicating an age-adjusted rate that was not much different from the slim subjects .
	manualset3
251685	6	426617	16	NULL	NULL	0	NULL	CHD events	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	During 16 years of follow-up of overweight subjects , 188 men and 44 women had CHD events , indicating an age-adjusted rate that was not much different from the slim subjects .
	manualset3
251686	7	426617	16	NULL	NULL	0	NULL	age-adjusted rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During 16 years of follow-up of overweight subjects , 188 men and 44 women had CHD events , indicating an age-adjusted rate that was not much different from the slim subjects .
	manualset3
251687	8	426617	16	NULL	NULL	0	NULL	slim subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	During 16 years of follow-up of overweight subjects , 188 men and 44 women had CHD events , indicating an age-adjusted rate that was not much different from the slim subjects .
	manualset3
251688	1	426618	16	NULL	NULL	0	NULL	2003	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	During 2003 , when the environmental study was undertaken , serotype O12 isolates with bla ( VIM ) were recovered from sinks and stethoscopes in the most-affected units , although not from the hands of staff ; the problem declined once these reservoirs were disinfected and hygienic precautions were reinforced .
	manualset3
251689	2	426618	16	NULL	NULL	0	NULL	environmental study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	During 2003 , when the environmental study was undertaken , serotype O12 isolates with bla ( VIM ) were recovered from sinks and stethoscopes in the most-affected units , although not from the hands of staff ; the problem declined once these reservoirs were disinfected and hygienic precautions were reinforced .
	manualset3
251690	3	426618	16	NULL	NULL	0	NULL	serotype O12 isolates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	During 2003 , when the environmental study was undertaken , serotype O12 isolates with bla ( VIM ) were recovered from sinks and stethoscopes in the most-affected units , although not from the hands of staff ; the problem declined once these reservoirs were disinfected and hygienic precautions were reinforced .
	manualset3
251691	4	426618	16	NULL	NULL	0	NULL	bla ( VIM )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	During 2003 , when the environmental study was undertaken , serotype O12 isolates with bla ( VIM ) were recovered from sinks and stethoscopes in the most-affected units , although not from the hands of staff ; the problem declined once these reservoirs were disinfected and hygienic precautions were reinforced .
	manualset3
251692	5	426618	16	NULL	NULL	0	NULL	sinks	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	During 2003 , when the environmental study was undertaken , serotype O12 isolates with bla ( VIM ) were recovered from sinks and stethoscopes in the most-affected units , although not from the hands of staff ; the problem declined once these reservoirs were disinfected and hygienic precautions were reinforced .
	manualset3
251693	6	426618	16	NULL	NULL	0	NULL	stethoscopes	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	During 2003 , when the environmental study was undertaken , serotype O12 isolates with bla ( VIM ) were recovered from sinks and stethoscopes in the most-affected units , although not from the hands of staff ; the problem declined once these reservoirs were disinfected and hygienic precautions were reinforced .
	manualset3
251694	7	426618	16	NULL	NULL	0	NULL	most-affected units	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	During 2003 , when the environmental study was undertaken , serotype O12 isolates with bla ( VIM ) were recovered from sinks and stethoscopes in the most-affected units , although not from the hands of staff ; the problem declined once these reservoirs were disinfected and hygienic precautions were reinforced .
	manualset3
251695	8	426618	16	NULL	NULL	0	NULL	hands	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	During 2003 , when the environmental study was undertaken , serotype O12 isolates with bla ( VIM ) were recovered from sinks and stethoscopes in the most-affected units , although not from the hands of staff ; the problem declined once these reservoirs were disinfected and hygienic precautions were reinforced .
	manualset3
251696	9	426618	16	NULL	NULL	0	NULL	staff	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	During 2003 , when the environmental study was undertaken , serotype O12 isolates with bla ( VIM ) were recovered from sinks and stethoscopes in the most-affected units , although not from the hands of staff ; the problem declined once these reservoirs were disinfected and hygienic precautions were reinforced .
	manualset3
251697	10	426618	16	NULL	NULL	0	NULL	problem	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	During 2003 , when the environmental study was undertaken , serotype O12 isolates with bla ( VIM ) were recovered from sinks and stethoscopes in the most-affected units , although not from the hands of staff ; the problem declined once these reservoirs were disinfected and hygienic precautions were reinforced .
	manualset3
251698	11	426618	16	NULL	NULL	0	NULL	reservoirs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	During 2003 , when the environmental study was undertaken , serotype O12 isolates with bla ( VIM ) were recovered from sinks and stethoscopes in the most-affected units , although not from the hands of staff ; the problem declined once these reservoirs were disinfected and hygienic precautions were reinforced .
	manualset3
251699	12	426618	16	NULL	NULL	0	NULL	hygienic precautions	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	During 2003 , when the environmental study was undertaken , serotype O12 isolates with bla ( VIM ) were recovered from sinks and stethoscopes in the most-affected units , although not from the hands of staff ; the problem declined once these reservoirs were disinfected and hygienic precautions were reinforced .
	manualset3
251700	1	426619	16	NULL	NULL	0	NULL	30 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	During 30 years of active participation in clinical vascular surgery and the screening and development of vascular prostheses , greater than 450 different fabrications have been evaluated .
	manualset3
251701	2	426619	16	NULL	NULL	0	NULL	participation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	During 30 years of active participation in clinical vascular surgery and the screening and development of vascular prostheses , greater than 450 different fabrications have been evaluated .
	manualset3
251702	3	426619	16	NULL	NULL	0	NULL	clinical vascular surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	During 30 years of active participation in clinical vascular surgery and the screening and development of vascular prostheses , greater than 450 different fabrications have been evaluated .
	manualset3
251703	4	426619	16	NULL	NULL	0	NULL	screening	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	During 30 years of active participation in clinical vascular surgery and the screening and development of vascular prostheses , greater than 450 different fabrications have been evaluated .
	manualset3
251704	5	426619	16	NULL	NULL	0	NULL	development	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	During 30 years of active participation in clinical vascular surgery and the screening and development of vascular prostheses , greater than 450 different fabrications have been evaluated .
	manualset3
251705	6	426619	16	NULL	NULL	0	NULL	vascular prostheses	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	During 30 years of active participation in clinical vascular surgery and the screening and development of vascular prostheses , greater than 450 different fabrications have been evaluated .
	manualset3
251706	7	426619	16	NULL	NULL	0	NULL	450	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	During 30 years of active participation in clinical vascular surgery and the screening and development of vascular prostheses , greater than 450 different fabrications have been evaluated .
	manualset3
251707	8	426619	16	NULL	NULL	0	NULL	fabrications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	During 30 years of active participation in clinical vascular surgery and the screening and development of vascular prostheses , greater than 450 different fabrications have been evaluated .
	manualset3
251708	1	426620	16	NULL	NULL	0	NULL	problems	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the problems of the married woman and the mother in nursing ) .
	manualset3
251709	2	426620	16	NULL	NULL	0	NULL	married woman	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the problems of the married woman and the mother in nursing ) .
	manualset3
251710	3	426620	16	NULL	NULL	0	NULL	mother	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the problems of the married woman and the mother in nursing ) .
	manualset3
251711	4	426620	16	NULL	NULL	0	NULL	nursing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the problems of the married woman and the mother in nursing ) .
	manualset3
251712	1	426621	16	NULL	NULL	0	NULL	CPB	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	During CPB and hemodilution , AI was correlated not only with Fb but also with haptoglobin and ceruloplasmin .
	manualset3
251713	2	426621	16	NULL	NULL	0	NULL	hemodilution	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	During CPB and hemodilution , AI was correlated not only with Fb but also with haptoglobin and ceruloplasmin .
	manualset3
251714	3	426621	16	NULL	NULL	0	NULL	AI	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During CPB and hemodilution , AI was correlated not only with Fb but also with haptoglobin and ceruloplasmin .
	manualset3
251715	4	426621	16	NULL	NULL	0	NULL	Fb	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	During CPB and hemodilution , AI was correlated not only with Fb but also with haptoglobin and ceruloplasmin .
	manualset3
251716	5	426621	16	NULL	NULL	0	NULL	haptoglobin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	During CPB and hemodilution , AI was correlated not only with Fb but also with haptoglobin and ceruloplasmin .
	manualset3
251717	6	426621	16	NULL	NULL	0	NULL	ceruloplasmin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	During CPB and hemodilution , AI was correlated not only with Fb but also with haptoglobin and ceruloplasmin .
	manualset3
251718	1	426622	16	NULL	NULL	0	NULL	June 2003	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	During June and July 2003 , CO , NO2 , THC and PM10 were sampled at the four highway toll gates in Chongqing .
	manualset3
251719	2	426622	16	NULL	NULL	0	NULL	July 2003	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	During June and July 2003 , CO , NO2 , THC and PM10 were sampled at the four highway toll gates in Chongqing .
	manualset3
251720	3	426622	16	NULL	NULL	0	NULL	CO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	During June and July 2003 , CO , NO2 , THC and PM10 were sampled at the four highway toll gates in Chongqing .
	manualset3
251721	4	426622	16	NULL	NULL	0	NULL	NO2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	During June and July 2003 , CO , NO2 , THC and PM10 were sampled at the four highway toll gates in Chongqing .
	manualset3
251722	5	426622	16	NULL	NULL	0	NULL	THC	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	During June and July 2003 , CO , NO2 , THC and PM10 were sampled at the four highway toll gates in Chongqing .
	manualset3
251723	6	426622	16	NULL	NULL	0	NULL	PM10	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	During June and July 2003 , CO , NO2 , THC and PM10 were sampled at the four highway toll gates in Chongqing .
	manualset3
251724	7	426622	16	NULL	NULL	0	NULL	four	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	During June and July 2003 , CO , NO2 , THC and PM10 were sampled at the four highway toll gates in Chongqing .
	manualset3
251725	8	426622	16	NULL	NULL	0	NULL	highway toll gates	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	During June and July 2003 , CO , NO2 , THC and PM10 were sampled at the four highway toll gates in Chongqing .
	manualset3
251726	9	426622	16	NULL	NULL	0	NULL	Chongqing	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	During June and July 2003 , CO , NO2 , THC and PM10 were sampled at the four highway toll gates in Chongqing .
	manualset3
251727	1	426623	16	NULL	NULL	0	NULL	SWS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	During SWS , body temperature is controlled by diencephalic structures whereas during REM sleep there is a suspension of hypothalamic thermoregulatory influences .
	manualset3
251728	2	426623	16	NULL	NULL	0	NULL	body temperature	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	During SWS , body temperature is controlled by diencephalic structures whereas during REM sleep there is a suspension of hypothalamic thermoregulatory influences .
	manualset3
251729	3	426623	16	NULL	NULL	0	NULL	diencephalic structures	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	During SWS , body temperature is controlled by diencephalic structures whereas during REM sleep there is a suspension of hypothalamic thermoregulatory influences .
	manualset3
251730	4	426623	16	NULL	NULL	0	NULL	REM sleep	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	During SWS , body temperature is controlled by diencephalic structures whereas during REM sleep there is a suspension of hypothalamic thermoregulatory influences .
	manualset3
251731	5	426623	16	NULL	NULL	0	NULL	suspension	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	During SWS , body temperature is controlled by diencephalic structures whereas during REM sleep there is a suspension of hypothalamic thermoregulatory influences .
	manualset3
251732	6	426623	16	NULL	NULL	0	NULL	hypothalamic thermoregulatory influences	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	During SWS , body temperature is controlled by diencephalic structures whereas during REM sleep there is a suspension of hypothalamic thermoregulatory influences .
	manualset3
251733	1	426624	16	NULL	NULL	0	NULL	follow-up interval	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	During a mean follow-up interval of 29 months , significant declines were detected in global cognitive ability ( d = .40 ) , visuoconstructive skills ( d = .32 ) , and memory ( d = .29 ) .
	manualset3
251734	2	426624	16	NULL	NULL	0	NULL	29 months	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	During a mean follow-up interval of 29 months , significant declines were detected in global cognitive ability ( d = .40 ) , visuoconstructive skills ( d = .32 ) , and memory ( d = .29 ) .
	manualset3
251735	3	426624	16	NULL	NULL	0	NULL	declines	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During a mean follow-up interval of 29 months , significant declines were detected in global cognitive ability ( d = .40 ) , visuoconstructive skills ( d = .32 ) , and memory ( d = .29 ) .
	manualset3
251736	4	426624	16	NULL	NULL	0	NULL	global cognitive ability	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	During a mean follow-up interval of 29 months , significant declines were detected in global cognitive ability ( d = .40 ) , visuoconstructive skills ( d = .32 ) , and memory ( d = .29 ) .
	manualset3
251737	5	426624	16	NULL	NULL	0	NULL	d = .40	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During a mean follow-up interval of 29 months , significant declines were detected in global cognitive ability ( d = .40 ) , visuoconstructive skills ( d = .32 ) , and memory ( d = .29 ) .
	manualset3
251738	6	426624	16	NULL	NULL	0	NULL	visuoconstructive skills	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	During a mean follow-up interval of 29 months , significant declines were detected in global cognitive ability ( d = .40 ) , visuoconstructive skills ( d = .32 ) , and memory ( d = .29 ) .
	manualset3
251739	7	426624	16	NULL	NULL	0	NULL	d = .32	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During a mean follow-up interval of 29 months , significant declines were detected in global cognitive ability ( d = .40 ) , visuoconstructive skills ( d = .32 ) , and memory ( d = .29 ) .
	manualset3
251740	8	426624	16	NULL	NULL	0	NULL	memory	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	During a mean follow-up interval of 29 months , significant declines were detected in global cognitive ability ( d = .40 ) , visuoconstructive skills ( d = .32 ) , and memory ( d = .29 ) .
	manualset3
251741	9	426624	16	NULL	NULL	0	NULL	d = .29	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During a mean follow-up interval of 29 months , significant declines were detected in global cognitive ability ( d = .40 ) , visuoconstructive skills ( d = .32 ) , and memory ( d = .29 ) .
	manualset3
251742	1	426625	16	NULL	NULL	0	NULL	mixed epidemic	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	During a mixed epidemic caused by the different strain of HA antigen , the infection ratio in mass population was revealed more convenient and sensitive by SRD than HAI .
	manualset3
251743	2	426625	16	NULL	NULL	0	NULL	strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	During a mixed epidemic caused by the different strain of HA antigen , the infection ratio in mass population was revealed more convenient and sensitive by SRD than HAI .
	manualset3
251744	3	426625	16	NULL	NULL	0	NULL	HA antigen	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	During a mixed epidemic caused by the different strain of HA antigen , the infection ratio in mass population was revealed more convenient and sensitive by SRD than HAI .
	manualset3
251745	4	426625	16	NULL	NULL	0	NULL	infection ratio	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During a mixed epidemic caused by the different strain of HA antigen , the infection ratio in mass population was revealed more convenient and sensitive by SRD than HAI .
	manualset3
251746	5	426625	16	NULL	NULL	0	NULL	mass population	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During a mixed epidemic caused by the different strain of HA antigen , the infection ratio in mass population was revealed more convenient and sensitive by SRD than HAI .
	manualset3
251747	6	426625	16	NULL	NULL	0	NULL	SRD	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	During a mixed epidemic caused by the different strain of HA antigen , the infection ratio in mass population was revealed more convenient and sensitive by SRD than HAI .
	manualset3
251748	7	426625	16	NULL	NULL	0	NULL	HAI	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	During a mixed epidemic caused by the different strain of HA antigen , the infection ratio in mass population was revealed more convenient and sensitive by SRD than HAI .
	manualset3
251749	1	426626	16	NULL	NULL	0	NULL	humoral factors	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	During a screen for humoral factors that promote cardiomyocyte differentiation from embryonic stem cells ( ESCs ) , we found marked elevation of granulocyte colony-stimulating factor receptor ( G-CSFR ) mRNA in developing cardiomyocytes .
	manualset3
251750	2	426626	16	NULL	NULL	0	NULL	cardiomyocyte differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	During a screen for humoral factors that promote cardiomyocyte differentiation from embryonic stem cells ( ESCs ) , we found marked elevation of granulocyte colony-stimulating factor receptor ( G-CSFR ) mRNA in developing cardiomyocytes .
	manualset3
251751	3	426626	16	NULL	NULL	0	NULL	embryonic stem cells ( ESCs )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	During a screen for humoral factors that promote cardiomyocyte differentiation from embryonic stem cells ( ESCs ) , we found marked elevation of granulocyte colony-stimulating factor receptor ( G-CSFR ) mRNA in developing cardiomyocytes .
	manualset3
251752	4	426626	16	NULL	NULL	0	NULL	elevation	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During a screen for humoral factors that promote cardiomyocyte differentiation from embryonic stem cells ( ESCs ) , we found marked elevation of granulocyte colony-stimulating factor receptor ( G-CSFR ) mRNA in developing cardiomyocytes .
	manualset3
251753	5	426626	16	NULL	NULL	0	NULL	granulocyte colony-stimulating factor receptor ( G-CSFR ) mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	During a screen for humoral factors that promote cardiomyocyte differentiation from embryonic stem cells ( ESCs ) , we found marked elevation of granulocyte colony-stimulating factor receptor ( G-CSFR ) mRNA in developing cardiomyocytes .
	manualset3
251754	6	426626	16	NULL	NULL	0	NULL	cardiomyocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	During a screen for humoral factors that promote cardiomyocyte differentiation from embryonic stem cells ( ESCs ) , we found marked elevation of granulocyte colony-stimulating factor receptor ( G-CSFR ) mRNA in developing cardiomyocytes .
	manualset3
251755	1	426627	16	NULL	NULL	0	NULL	therapeutic use	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the therapeutic use of sulfoniazid in tuberculosis ) .
	manualset3
251756	2	426627	16	NULL	NULL	0	NULL	sulfoniazid	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the therapeutic use of sulfoniazid in tuberculosis ) .
	manualset3
251757	3	426627	16	NULL	NULL	0	NULL	tuberculosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the therapeutic use of sulfoniazid in tuberculosis ) .
	manualset3
251758	1	426628	16	NULL	NULL	0	NULL	follow-up	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	During a total follow-up of 7.4 + / - 2.2 years there were no differences in the incidence of clinical variables as compared to age-matched controls with DDD pacemakers .
	manualset3
251759	2	426628	16	NULL	NULL	0	NULL	7.4 + / - 2.2 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	During a total follow-up of 7.4 + / - 2.2 years there were no differences in the incidence of clinical variables as compared to age-matched controls with DDD pacemakers .
	manualset3
251760	3	426628	16	NULL	NULL	0	NULL	differences	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During a total follow-up of 7.4 + / - 2.2 years there were no differences in the incidence of clinical variables as compared to age-matched controls with DDD pacemakers .
	manualset3
251761	4	426628	16	NULL	NULL	0	NULL	incidence	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During a total follow-up of 7.4 + / - 2.2 years there were no differences in the incidence of clinical variables as compared to age-matched controls with DDD pacemakers .
	manualset3
251762	5	426628	16	NULL	NULL	0	NULL	clinical variables	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	During a total follow-up of 7.4 + / - 2.2 years there were no differences in the incidence of clinical variables as compared to age-matched controls with DDD pacemakers .
	manualset3
251763	6	426628	16	NULL	NULL	0	NULL	age-matched controls	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	During a total follow-up of 7.4 + / - 2.2 years there were no differences in the incidence of clinical variables as compared to age-matched controls with DDD pacemakers .
	manualset3
251764	7	426628	16	NULL	NULL	0	NULL	DDD pacemakers	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	During a total follow-up of 7.4 + / - 2.2 years there were no differences in the incidence of clinical variables as compared to age-matched controls with DDD pacemakers .
	manualset3
251765	1	426629	16	NULL	NULL	0	NULL	experimental procedure	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	During all the experimental procedure , the animals were maintained under 1-h limited access to alcohol .
	manualset3
251766	2	426629	16	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	During all the experimental procedure , the animals were maintained under 1-h limited access to alcohol .
	manualset3
251767	3	426629	16	NULL	NULL	0	NULL	1-h limited access	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	During all the experimental procedure , the animals were maintained under 1-h limited access to alcohol .
	manualset3
251768	4	426629	16	NULL	NULL	0	NULL	alcohol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	During all the experimental procedure , the animals were maintained under 1-h limited access to alcohol .
	manualset3
251769	1	426630	16	NULL	NULL	0	NULL	anaesthesia	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	During anaesthesia , , left bundle branch block may be related to hypertension or tachycardia and its occurrence makes the diagnosis of acute myocardial ischemia or infarction difficult .
	manualset3
251770	2	426630	16	NULL	NULL	0	NULL	left bundle branch block	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	During anaesthesia , , left bundle branch block may be related to hypertension or tachycardia and its occurrence makes the diagnosis of acute myocardial ischemia or infarction difficult .
	manualset3
251771	3	426630	16	NULL	NULL	0	NULL	hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	During anaesthesia , , left bundle branch block may be related to hypertension or tachycardia and its occurrence makes the diagnosis of acute myocardial ischemia or infarction difficult .
	manualset3
251772	4	426630	16	NULL	NULL	0	NULL	tachycardia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	During anaesthesia , , left bundle branch block may be related to hypertension or tachycardia and its occurrence makes the diagnosis of acute myocardial ischemia or infarction difficult .
	manualset3
251773	5	426630	16	NULL	NULL	0	NULL	occurrence	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During anaesthesia , , left bundle branch block may be related to hypertension or tachycardia and its occurrence makes the diagnosis of acute myocardial ischemia or infarction difficult .
	manualset3
251774	6	426630	16	NULL	NULL	0	NULL	diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	During anaesthesia , , left bundle branch block may be related to hypertension or tachycardia and its occurrence makes the diagnosis of acute myocardial ischemia or infarction difficult .
	manualset3
251775	7	426630	16	NULL	NULL	0	NULL	acute myocardial ischemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	During anaesthesia , , left bundle branch block may be related to hypertension or tachycardia and its occurrence makes the diagnosis of acute myocardial ischemia or infarction difficult .
	manualset3
251776	8	426630	16	NULL	NULL	0	NULL	acute myocardial infarction	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	During anaesthesia , , left bundle branch block may be related to hypertension or tachycardia and its occurrence makes the diagnosis of acute myocardial ischemia or infarction difficult .
	manualset3
251777	1	426631	16	NULL	NULL	0	NULL	bacterial peritonitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	During bacterial peritonitis of patients on continuous ambulatory peritoneal dialysis ( CAPD ) leukocytes , particularly polymorphonuclear neutrophilic granulocytes ( PMNs ) , migrate into the peritoneal cavity .
	manualset3
251778	2	426631	16	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	During bacterial peritonitis of patients on continuous ambulatory peritoneal dialysis ( CAPD ) leukocytes , particularly polymorphonuclear neutrophilic granulocytes ( PMNs ) , migrate into the peritoneal cavity .
	manualset3
251779	3	426631	16	NULL	NULL	0	NULL	continuous ambulatory peritoneal dialysis ( CAPD )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	During bacterial peritonitis of patients on continuous ambulatory peritoneal dialysis ( CAPD ) leukocytes , particularly polymorphonuclear neutrophilic granulocytes ( PMNs ) , migrate into the peritoneal cavity .
	manualset3
251780	4	426631	16	NULL	NULL	0	NULL	leukocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	During bacterial peritonitis of patients on continuous ambulatory peritoneal dialysis ( CAPD ) leukocytes , particularly polymorphonuclear neutrophilic granulocytes ( PMNs ) , migrate into the peritoneal cavity .
	manualset3
251781	5	426631	16	NULL	NULL	0	NULL	polymorphonuclear neutrophilic granulocytes ( PMNs )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	During bacterial peritonitis of patients on continuous ambulatory peritoneal dialysis ( CAPD ) leukocytes , particularly polymorphonuclear neutrophilic granulocytes ( PMNs ) , migrate into the peritoneal cavity .
	manualset3
251782	6	426631	16	NULL	NULL	0	NULL	peritoneal cavity	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	During bacterial peritonitis of patients on continuous ambulatory peritoneal dialysis ( CAPD ) leukocytes , particularly polymorphonuclear neutrophilic granulocytes ( PMNs ) , migrate into the peritoneal cavity .
	manualset3
251783	1	426632	16	NULL	NULL	0	NULL	conditions	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	During both conditions , however , there were similar increases of accuracy scores .
	manualset3
251784	2	426632	16	NULL	NULL	0	NULL	increases	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	During both conditions , however , there were similar increases of accuracy scores .
	manualset3
251785	3	426632	16	NULL	NULL	0	NULL	accuracy scores	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During both conditions , however , there were similar increases of accuracy scores .
	manualset3
251786	1	426633	16	NULL	NULL	0	NULL	cardiopulmonary bypass	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	During cardiopulmonary bypass the mean fluorescence values for glycoprotein llla , GMP-33 , and the percentage of GMP-140 and lysosome integral membrane protein-CD63 expressing platelets increased significantly .
	manualset3
251787	2	426633	16	NULL	NULL	0	NULL	fluorescence values	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During cardiopulmonary bypass the mean fluorescence values for glycoprotein llla , GMP-33 , and the percentage of GMP-140 and lysosome integral membrane protein-CD63 expressing platelets increased significantly .
	manualset3
251788	3	426633	16	NULL	NULL	0	NULL	glycoprotein llla	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	During cardiopulmonary bypass the mean fluorescence values for glycoprotein llla , GMP-33 , and the percentage of GMP-140 and lysosome integral membrane protein-CD63 expressing platelets increased significantly .
	manualset3
251789	4	426633	16	NULL	NULL	0	NULL	GMP-33	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	During cardiopulmonary bypass the mean fluorescence values for glycoprotein llla , GMP-33 , and the percentage of GMP-140 and lysosome integral membrane protein-CD63 expressing platelets increased significantly .
	manualset3
251790	5	426633	16	NULL	NULL	0	NULL	percentage	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During cardiopulmonary bypass the mean fluorescence values for glycoprotein llla , GMP-33 , and the percentage of GMP-140 and lysosome integral membrane protein-CD63 expressing platelets increased significantly .
	manualset3
251791	6	426633	16	NULL	NULL	0	NULL	GMP-140	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	During cardiopulmonary bypass the mean fluorescence values for glycoprotein llla , GMP-33 , and the percentage of GMP-140 and lysosome integral membrane protein-CD63 expressing platelets increased significantly .
	manualset3
251792	7	426633	16	NULL	NULL	0	NULL	lysosome integral membrane protein-CD63	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	During cardiopulmonary bypass the mean fluorescence values for glycoprotein llla , GMP-33 , and the percentage of GMP-140 and lysosome integral membrane protein-CD63 expressing platelets increased significantly .
	manualset3
251793	8	426633	16	NULL	NULL	0	NULL	platelets	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	During cardiopulmonary bypass the mean fluorescence values for glycoprotein llla , GMP-33 , and the percentage of GMP-140 and lysosome integral membrane protein-CD63 expressing platelets increased significantly .
	manualset3
252037	1	426634	16	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	During development , Dlx3 is expressed in ectodermal appendages such as hair and teeth .
	manualset3
252038	2	426634	16	NULL	NULL	0	NULL	Dlx3	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	During development , Dlx3 is expressed in ectodermal appendages such as hair and teeth .
	manualset3
252039	3	426634	16	NULL	NULL	0	NULL	ectodermal appendages	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	During development , Dlx3 is expressed in ectodermal appendages such as hair and teeth .
	manualset3
252040	4	426634	16	NULL	NULL	0	NULL	hair	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	During development , Dlx3 is expressed in ectodermal appendages such as hair and teeth .
	manualset3
252041	5	426634	16	NULL	NULL	0	NULL	teeth	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	During development , Dlx3 is expressed in ectodermal appendages such as hair and teeth .
	manualset3
252042	1	426635	16	NULL	NULL	0	NULL	treatment	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the treatment of vitiligo with Ammi majus ) .
	manualset3
252043	2	426635	16	NULL	NULL	0	NULL	vitiligo	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the treatment of vitiligo with Ammi majus ) .
	manualset3
252044	3	426635	16	NULL	NULL	0	NULL	Ammi majus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( On the treatment of vitiligo with Ammi majus ) .
	manualset3
252045	1	426636	16	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	During development endothelial cells ` invade ' the retina , accompanied by a population of microglial cells ; glial fibrillary acidic protein ( GFAP ) - immunoreactive astrocytes are also seen associated with the developing vasculature , and are in advance of the vascular front by a few hundred microns .
	manualset3
252046	2	426636	16	NULL	NULL	0	NULL	endothelial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	During development endothelial cells ` invade ' the retina , accompanied by a population of microglial cells ; glial fibrillary acidic protein ( GFAP ) - immunoreactive astrocytes are also seen associated with the developing vasculature , and are in advance of the vascular front by a few hundred microns .
	manualset3
252047	3	426636	16	NULL	NULL	0	NULL	retina	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	During development endothelial cells ` invade ' the retina , accompanied by a population of microglial cells ; glial fibrillary acidic protein ( GFAP ) - immunoreactive astrocytes are also seen associated with the developing vasculature , and are in advance of the vascular front by a few hundred microns .
	manualset3
252048	4	426636	16	NULL	NULL	0	NULL	population	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During development endothelial cells ` invade ' the retina , accompanied by a population of microglial cells ; glial fibrillary acidic protein ( GFAP ) - immunoreactive astrocytes are also seen associated with the developing vasculature , and are in advance of the vascular front by a few hundred microns .
	manualset3
252049	5	426636	16	NULL	NULL	0	NULL	microglial cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	During development endothelial cells ` invade ' the retina , accompanied by a population of microglial cells ; glial fibrillary acidic protein ( GFAP ) - immunoreactive astrocytes are also seen associated with the developing vasculature , and are in advance of the vascular front by a few hundred microns .
	manualset3
252050	6	426636	16	NULL	NULL	0	NULL	glial fibrillary acidic protein ( GFAP )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	During development endothelial cells ` invade ' the retina , accompanied by a population of microglial cells ; glial fibrillary acidic protein ( GFAP ) - immunoreactive astrocytes are also seen associated with the developing vasculature , and are in advance of the vascular front by a few hundred microns .
	manualset3
252051	7	426636	16	NULL	NULL	0	NULL	immunoreactive astrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	During development endothelial cells ` invade ' the retina , accompanied by a population of microglial cells ; glial fibrillary acidic protein ( GFAP ) - immunoreactive astrocytes are also seen associated with the developing vasculature , and are in advance of the vascular front by a few hundred microns .
	manualset3
252052	8	426636	16	NULL	NULL	0	NULL	vasculature	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	During development endothelial cells ` invade ' the retina , accompanied by a population of microglial cells ; glial fibrillary acidic protein ( GFAP ) - immunoreactive astrocytes are also seen associated with the developing vasculature , and are in advance of the vascular front by a few hundred microns .
	manualset3
252053	9	426636	16	NULL	NULL	0	NULL	vascular front	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	During development endothelial cells ` invade ' the retina , accompanied by a population of microglial cells ; glial fibrillary acidic protein ( GFAP ) - immunoreactive astrocytes are also seen associated with the developing vasculature , and are in advance of the vascular front by a few hundred microns .
	manualset3
252054	10	426636	16	NULL	NULL	0	NULL	few hundred microns	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During development endothelial cells ` invade ' the retina , accompanied by a population of microglial cells ; glial fibrillary acidic protein ( GFAP ) - immunoreactive astrocytes are also seen associated with the developing vasculature , and are in advance of the vascular front by a few hundred microns .
	manualset3
252055	1	426637	16	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	During development from the embryo to the adult , a progressive increase in ploidy classes associated with an enhancement of megakaryocyte ( meg ) size was observed .
	manualset3
252056	2	426637	16	NULL	NULL	0	NULL	embryo	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	During development from the embryo to the adult , a progressive increase in ploidy classes associated with an enhancement of megakaryocyte ( meg ) size was observed .
	manualset3
252057	3	426637	16	NULL	NULL	0	NULL	adult	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	During development from the embryo to the adult , a progressive increase in ploidy classes associated with an enhancement of megakaryocyte ( meg ) size was observed .
	manualset3
252058	4	426637	16	NULL	NULL	0	NULL	progressive increase	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During development from the embryo to the adult , a progressive increase in ploidy classes associated with an enhancement of megakaryocyte ( meg ) size was observed .
	manualset3
252059	5	426637	16	NULL	NULL	0	NULL	ploidy classes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	During development from the embryo to the adult , a progressive increase in ploidy classes associated with an enhancement of megakaryocyte ( meg ) size was observed .
	manualset3
252060	6	426637	16	NULL	NULL	0	NULL	enhancement	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During development from the embryo to the adult , a progressive increase in ploidy classes associated with an enhancement of megakaryocyte ( meg ) size was observed .
	manualset3
252061	7	426637	16	NULL	NULL	0	NULL	 megakaryocyte ( meg )	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	During development from the embryo to the adult , a progressive increase in ploidy classes associated with an enhancement of megakaryocyte ( meg ) size was observed .
	manualset3
252062	8	426637	16	NULL	NULL	0	NULL	size	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During development from the embryo to the adult , a progressive increase in ploidy classes associated with an enhancement of megakaryocyte ( meg ) size was observed .
	manualset3
252063	1	426638	16	NULL	NULL	0	NULL	development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	During development of the somatic macronucleus from the germline micronucleus in ciliates , chromosome rearrangements occur in which specific regions of DNA are eliminated and flanking regions are healed , either by religation or construction of telomeres .
	manualset3
252064	2	426638	16	NULL	NULL	0	NULL	somatic macronucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	During development of the somatic macronucleus from the germline micronucleus in ciliates , chromosome rearrangements occur in which specific regions of DNA are eliminated and flanking regions are healed , either by religation or construction of telomeres .
	manualset3
252065	3	426638	16	NULL	NULL	0	NULL	germline micronucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	During development of the somatic macronucleus from the germline micronucleus in ciliates , chromosome rearrangements occur in which specific regions of DNA are eliminated and flanking regions are healed , either by religation or construction of telomeres .
	manualset3
252066	4	426638	16	NULL	NULL	0	NULL	ciliates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	During development of the somatic macronucleus from the germline micronucleus in ciliates , chromosome rearrangements occur in which specific regions of DNA are eliminated and flanking regions are healed , either by religation or construction of telomeres .
	manualset3
252067	5	426638	16	NULL	NULL	0	NULL	chromosome rearrangements	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	During development of the somatic macronucleus from the germline micronucleus in ciliates , chromosome rearrangements occur in which specific regions of DNA are eliminated and flanking regions are healed , either by religation or construction of telomeres .
	manualset3
252068	6	426638	16	NULL	NULL	0	NULL	regions of DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	During development of the somatic macronucleus from the germline micronucleus in ciliates , chromosome rearrangements occur in which specific regions of DNA are eliminated and flanking regions are healed , either by religation or construction of telomeres .
	manualset3
252069	7	426638	16	NULL	NULL	0	NULL	flanking regions	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	During development of the somatic macronucleus from the germline micronucleus in ciliates , chromosome rearrangements occur in which specific regions of DNA are eliminated and flanking regions are healed , either by religation or construction of telomeres .
	manualset3
252070	8	426638	16	NULL	NULL	0	NULL	religation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	During development of the somatic macronucleus from the germline micronucleus in ciliates , chromosome rearrangements occur in which specific regions of DNA are eliminated and flanking regions are healed , either by religation or construction of telomeres .
	manualset3
252071	9	426638	16	NULL	NULL	0	NULL	construction of telomeres	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	During development of the somatic macronucleus from the germline micronucleus in ciliates , chromosome rearrangements occur in which specific regions of DNA are eliminated and flanking regions are healed , either by religation or construction of telomeres .
	manualset3
252072	1	426639	16	NULL	NULL	0	NULL	differentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	During differentiation of cytotrophoblast cells to syncytiotrophoblasts , IGF-I binding capacity increased 40 per cent from 80 to 130 fmol/mg protein on day 1 to day 2 , then decreased by 70 per cent from 130 to 40 fmol/mg protein on day 2 to day 3 .
	manualset3
252073	2	426639	16	NULL	NULL	0	NULL	cytotrophoblast cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	During differentiation of cytotrophoblast cells to syncytiotrophoblasts , IGF-I binding capacity increased 40 per cent from 80 to 130 fmol/mg protein on day 1 to day 2 , then decreased by 70 per cent from 130 to 40 fmol/mg protein on day 2 to day 3 .
	manualset3
252084	3	426639	16	NULL	NULL	0	NULL	syncytiotrophoblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	During differentiation of cytotrophoblast cells to syncytiotrophoblasts , IGF-I binding capacity increased 40 per cent from 80 to 130 fmol/mg protein on day 1 to day 2 , then decreased by 70 per cent from 130 to 40 fmol/mg protein on day 2 to day 3 .
	manualset3
252085	4	426639	16	NULL	NULL	0	NULL	IGF-I binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	During differentiation of cytotrophoblast cells to syncytiotrophoblasts , IGF-I binding capacity increased 40 per cent from 80 to 130 fmol/mg protein on day 1 to day 2 , then decreased by 70 per cent from 130 to 40 fmol/mg protein on day 2 to day 3 .
	manualset3
252086	5	426639	16	NULL	NULL	0	NULL	capacity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During differentiation of cytotrophoblast cells to syncytiotrophoblasts , IGF-I binding capacity increased 40 per cent from 80 to 130 fmol/mg protein on day 1 to day 2 , then decreased by 70 per cent from 130 to 40 fmol/mg protein on day 2 to day 3 .
	manualset3
252087	6	426639	16	NULL	NULL	0	NULL	40 per cent	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During differentiation of cytotrophoblast cells to syncytiotrophoblasts , IGF-I binding capacity increased 40 per cent from 80 to 130 fmol/mg protein on day 1 to day 2 , then decreased by 70 per cent from 130 to 40 fmol/mg protein on day 2 to day 3 .
	manualset3
252088	7	426639	16	NULL	NULL	0	NULL	80 to 130 fmol/mg protein	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During differentiation of cytotrophoblast cells to syncytiotrophoblasts , IGF-I binding capacity increased 40 per cent from 80 to 130 fmol/mg protein on day 1 to day 2 , then decreased by 70 per cent from 130 to 40 fmol/mg protein on day 2 to day 3 .
	manualset3
252089	8	426639	16	NULL	NULL	0	NULL	day 1 to day 2	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	During differentiation of cytotrophoblast cells to syncytiotrophoblasts , IGF-I binding capacity increased 40 per cent from 80 to 130 fmol/mg protein on day 1 to day 2 , then decreased by 70 per cent from 130 to 40 fmol/mg protein on day 2 to day 3 .
	manualset3
252090	9	426639	16	NULL	NULL	0	NULL	70 per cent	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During differentiation of cytotrophoblast cells to syncytiotrophoblasts , IGF-I binding capacity increased 40 per cent from 80 to 130 fmol/mg protein on day 1 to day 2 , then decreased by 70 per cent from 130 to 40 fmol/mg protein on day 2 to day 3 .
	manualset3
252091	10	426639	16	NULL	NULL	0	NULL	130 to 40 fmol/mg protein	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During differentiation of cytotrophoblast cells to syncytiotrophoblasts , IGF-I binding capacity increased 40 per cent from 80 to 130 fmol/mg protein on day 1 to day 2 , then decreased by 70 per cent from 130 to 40 fmol/mg protein on day 2 to day 3 .
	manualset3
252092	11	426639	16	NULL	NULL	0	NULL	day 2 to day 3	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	During differentiation of cytotrophoblast cells to syncytiotrophoblasts , IGF-I binding capacity increased 40 per cent from 80 to 130 fmol/mg protein on day 1 to day 2 , then decreased by 70 per cent from 130 to 40 fmol/mg protein on day 2 to day 3 .
	manualset3
252093	1	426640	16	NULL	NULL	0	NULL	drowsiness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	During drowsiness , no separate mismatch negativity ( MMN ) could be detected , but the 2000 Hz tone evoked a broad fronto-central early negative deflection , suggesting an overlap of N1 and MMN .
	manualset3
252094	2	426640	16	NULL	NULL	0	NULL	no separate mismatch negativity ( MMN )	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	During drowsiness , no separate mismatch negativity ( MMN ) could be detected , but the 2000 Hz tone evoked a broad fronto-central early negative deflection , suggesting an overlap of N1 and MMN .
	manualset3
252095	3	426640	16	NULL	NULL	0	NULL	2000 Hz tone	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During drowsiness , no separate mismatch negativity ( MMN ) could be detected , but the 2000 Hz tone evoked a broad fronto-central early negative deflection , suggesting an overlap of N1 and MMN .
	manualset3
252096	4	426640	16	NULL	NULL	NULL	NULL	broad fronto-central early negative deflection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During drowsiness , no separate mismatch negativity ( MMN ) could be detected , but the 2000 Hz tone evoked a broad fronto-central early negative deflection , suggesting an overlap of N1 and MMN .
	manualset3
252097	5	426640	16	NULL	NULL	0	NULL	overlap	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During drowsiness , no separate mismatch negativity ( MMN ) could be detected , but the 2000 Hz tone evoked a broad fronto-central early negative deflection , suggesting an overlap of N1 and MMN .
	manualset3
252100	6	426640	16	NULL	NULL	0	NULL	N1	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	During drowsiness , no separate mismatch negativity ( MMN ) could be detected , but the 2000 Hz tone evoked a broad fronto-central early negative deflection , suggesting an overlap of N1 and MMN .
	manualset3
252101	7	426640	16	NULL	NULL	0	NULL	MMN	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	During drowsiness , no separate mismatch negativity ( MMN ) could be detected , but the 2000 Hz tone evoked a broad fronto-central early negative deflection , suggesting an overlap of N1 and MMN .
	manualset3
252108	1	426641	16	NULL	NULL	0	NULL	mammalian development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	During early mammalian development , as the pluripotent cells that give rise to all of the tissues of the body proliferate and expand in number , they pass through transition states marked by a stepwise restriction in developmental potential and by changes in the expression of key regulatory genes .
	manualset3
252109	2	426641	16	NULL	NULL	0	NULL	pluripotent cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	During early mammalian development , as the pluripotent cells that give rise to all of the tissues of the body proliferate and expand in number , they pass through transition states marked by a stepwise restriction in developmental potential and by changes in the expression of key regulatory genes .
	manualset3
252111	3	426641	16	NULL	NULL	0	NULL	tissues	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	During early mammalian development , as the pluripotent cells that give rise to all of the tissues of the body proliferate and expand in number , they pass through transition states marked by a stepwise restriction in developmental potential and by changes in the expression of key regulatory genes .
	manualset3
252112	4	426641	16	NULL	NULL	NULL	NULL	body	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During early mammalian development , as the pluripotent cells that give rise to all of the tissues of the body proliferate and expand in number , they pass through transition states marked by a stepwise restriction in developmental potential and by changes in the expression of key regulatory genes .
	manualset3
252113	5	426641	16	NULL	NULL	0	NULL	number	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During early mammalian development , as the pluripotent cells that give rise to all of the tissues of the body proliferate and expand in number , they pass through transition states marked by a stepwise restriction in developmental potential and by changes in the expression of key regulatory genes .
	manualset3
252115	6	426641	16	NULL	NULL	0	NULL	transition states	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	During early mammalian development , as the pluripotent cells that give rise to all of the tissues of the body proliferate and expand in number , they pass through transition states marked by a stepwise restriction in developmental potential and by changes in the expression of key regulatory genes .
	manualset3
252116	7	426641	16	NULL	NULL	0	NULL	restriction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	During early mammalian development , as the pluripotent cells that give rise to all of the tissues of the body proliferate and expand in number , they pass through transition states marked by a stepwise restriction in developmental potential and by changes in the expression of key regulatory genes .
	manualset3
252117	8	426641	16	NULL	NULL	0	NULL	developmental potential	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During early mammalian development , as the pluripotent cells that give rise to all of the tissues of the body proliferate and expand in number , they pass through transition states marked by a stepwise restriction in developmental potential and by changes in the expression of key regulatory genes .
	manualset3
252118	9	426641	16	NULL	NULL	0	NULL	changes	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	During early mammalian development , as the pluripotent cells that give rise to all of the tissues of the body proliferate and expand in number , they pass through transition states marked by a stepwise restriction in developmental potential and by changes in the expression of key regulatory genes .
	manualset3
252119	10	426641	16	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	During early mammalian development , as the pluripotent cells that give rise to all of the tissues of the body proliferate and expand in number , they pass through transition states marked by a stepwise restriction in developmental potential and by changes in the expression of key regulatory genes .
	manualset3
252120	11	426641	16	NULL	NULL	0	NULL	key regulatory genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	During early mammalian development , as the pluripotent cells that give rise to all of the tissues of the body proliferate and expand in number , they pass through transition states marked by a stepwise restriction in developmental potential and by changes in the expression of key regulatory genes .
	manualset3
252125	1	426642	16	NULL	NULL	0	NULL	 embryonic brain development	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	During embryonic brain development of Drosophila , the Hox gene labial ( lab ) is essential for tritocerebral neuromere specification ; lab loss of function results in tritocerebral cells that fail to adopt a neuronal identity , causing axonal pathfinding defects .
	manualset3
252126	2	426642	16	NULL	NULL	0	NULL	Drosophila	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	During embryonic brain development of Drosophila , the Hox gene labial ( lab ) is essential for tritocerebral neuromere specification ; lab loss of function results in tritocerebral cells that fail to adopt a neuronal identity , causing axonal pathfinding defects .
	manualset3
252127	3	426642	16	NULL	NULL	0	NULL	Hox gene labial ( lab )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	During embryonic brain development of Drosophila , the Hox gene labial ( lab ) is essential for tritocerebral neuromere specification ; lab loss of function results in tritocerebral cells that fail to adopt a neuronal identity , causing axonal pathfinding defects .
	manualset3
252133	4	426642	16	NULL	NULL	0	NULL	tritocerebral neuromere specification	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	During embryonic brain development of Drosophila , the Hox gene labial ( lab ) is essential for tritocerebral neuromere specification ; lab loss of function results in tritocerebral cells that fail to adopt a neuronal identity , causing axonal pathfinding defects .
	manualset3
252136	5	426642	16	NULL	NULL	0	NULL	lab loss of function	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	During embryonic brain development of Drosophila , the Hox gene labial ( lab ) is essential for tritocerebral neuromere specification ; lab loss of function results in tritocerebral cells that fail to adopt a neuronal identity , causing axonal pathfinding defects .
	manualset3
252140	6	426642	16	NULL	NULL	NULL	NULL	results	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During embryonic brain development of Drosophila , the Hox gene labial ( lab ) is essential for tritocerebral neuromere specification ; lab loss of function results in tritocerebral cells that fail to adopt a neuronal identity , causing axonal pathfinding defects .
	manualset3
252142	7	426642	16	NULL	NULL	0	NULL	tritocerebral cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	During embryonic brain development of Drosophila , the Hox gene labial ( lab ) is essential for tritocerebral neuromere specification ; lab loss of function results in tritocerebral cells that fail to adopt a neuronal identity , causing axonal pathfinding defects .
	manualset3
252143	8	426642	16	NULL	NULL	0	NULL	neuronal identity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	During embryonic brain development of Drosophila , the Hox gene labial ( lab ) is essential for tritocerebral neuromere specification ; lab loss of function results in tritocerebral cells that fail to adopt a neuronal identity , causing axonal pathfinding defects .
	manualset3
252144	8	426642	16	NULL	NULL	NULL	NULL	axonal pathfinding defects	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During embryonic brain development of Drosophila , the Hox gene labial ( lab ) is essential for tritocerebral neuromere specification ; lab loss of function results in tritocerebral cells that fail to adopt a neuronal identity , causing axonal pathfinding defects .
	manualset3
255847	1	426643	16	NULL	NULL	NULL	NULL	endovideoscopy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During endovideoscopy of the residual cavities the remnants of the chitinous membranes and small daughter vesicles not noticed during the open stage of the operation were removed in 7.4 % of the patients , in 25.9 % of the patients cystobiliary fistulas were detected .
	manualset3
256273	2	426643	16	NULL	NULL	NULL	NULL	residual cavities	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During endovideoscopy of the residual cavities the remnants of the chitinous membranes and small daughter vesicles not noticed during the open stage of the operation were removed in 7.4 % of the patients , in 25.9 % of the patients cystobiliary fistulas were detected .
	manualset3
256274	3	426643	16	NULL	NULL	NULL	NULL	remnants	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During endovideoscopy of the residual cavities the remnants of the chitinous membranes and small daughter vesicles not noticed during the open stage of the operation were removed in 7.4 % of the patients , in 25.9 % of the patients cystobiliary fistulas were detected .
	manualset3
256275	4	426643	16	NULL	NULL	NULL	NULL	chitinous membranes	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During endovideoscopy of the residual cavities the remnants of the chitinous membranes and small daughter vesicles not noticed during the open stage of the operation were removed in 7.4 % of the patients , in 25.9 % of the patients cystobiliary fistulas were detected .
	manualset3
256276	5	426643	16	NULL	NULL	NULL	NULL	small daughter vesicles	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During endovideoscopy of the residual cavities the remnants of the chitinous membranes and small daughter vesicles not noticed during the open stage of the operation were removed in 7.4 % of the patients , in 25.9 % of the patients cystobiliary fistulas were detected .
	manualset3
256277	6	426643	16	NULL	NULL	NULL	NULL	open stage	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During endovideoscopy of the residual cavities the remnants of the chitinous membranes and small daughter vesicles not noticed during the open stage of the operation were removed in 7.4 % of the patients , in 25.9 % of the patients cystobiliary fistulas were detected .
	manualset3
256278	7	426643	16	NULL	NULL	NULL	NULL	operation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During endovideoscopy of the residual cavities the remnants of the chitinous membranes and small daughter vesicles not noticed during the open stage of the operation were removed in 7.4 % of the patients , in 25.9 % of the patients cystobiliary fistulas were detected .
	manualset3
256279	8	426643	16	NULL	NULL	NULL	NULL	7.4 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During endovideoscopy of the residual cavities the remnants of the chitinous membranes and small daughter vesicles not noticed during the open stage of the operation were removed in 7.4 % of the patients , in 25.9 % of the patients cystobiliary fistulas were detected .
	manualset3
256280	9	426643	16	NULL	NULL	NULL	NULL	 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During endovideoscopy of the residual cavities the remnants of the chitinous membranes and small daughter vesicles not noticed during the open stage of the operation were removed in 7.4 % of the patients , in 25.9 % of the patients cystobiliary fistulas were detected .
	manualset3
256281	10	426643	16	NULL	NULL	NULL	NULL	25.9 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During endovideoscopy of the residual cavities the remnants of the chitinous membranes and small daughter vesicles not noticed during the open stage of the operation were removed in 7.4 % of the patients , in 25.9 % of the patients cystobiliary fistulas were detected .
	manualset3
256282	11	426643	16	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During endovideoscopy of the residual cavities the remnants of the chitinous membranes and small daughter vesicles not noticed during the open stage of the operation were removed in 7.4 % of the patients , in 25.9 % of the patients cystobiliary fistulas were detected .
	manualset3
256283	12	426643	16	NULL	NULL	NULL	NULL	cystobiliary fistulas	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During endovideoscopy of the residual cavities the remnants of the chitinous membranes and small daughter vesicles not noticed during the open stage of the operation were removed in 7.4 % of the patients , in 25.9 % of the patients cystobiliary fistulas were detected .
	manualset3
256284	1	426644	16	NULL	NULL	NULL	NULL	exocytosis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During exocytosis of the dense vesicles an electron dense material is released which coalesces with the surface coat of the ovum to form a thin hatching envelope which eventually lifts from the ovum 's surface .
	manualset3
256285	2	426644	16	NULL	NULL	NULL	NULL	dense vesicles	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During exocytosis of the dense vesicles an electron dense material is released which coalesces with the surface coat of the ovum to form a thin hatching envelope which eventually lifts from the ovum 's surface .
	manualset3
256286	3	426644	16	NULL	NULL	NULL	NULL	electron dense material	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During exocytosis of the dense vesicles an electron dense material is released which coalesces with the surface coat of the ovum to form a thin hatching envelope which eventually lifts from the ovum 's surface .
	manualset3
256287	4	426644	16	NULL	NULL	NULL	NULL	surface coat	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During exocytosis of the dense vesicles an electron dense material is released which coalesces with the surface coat of the ovum to form a thin hatching envelope which eventually lifts from the ovum 's surface .
	manualset3
256288	5	426644	16	NULL	NULL	NULL	NULL	ovum	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During exocytosis of the dense vesicles an electron dense material is released which coalesces with the surface coat of the ovum to form a thin hatching envelope which eventually lifts from the ovum 's surface .
	manualset3
256289	6	426644	16	NULL	NULL	NULL	NULL	thin hatching envelope	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During exocytosis of the dense vesicles an electron dense material is released which coalesces with the surface coat of the ovum to form a thin hatching envelope which eventually lifts from the ovum 's surface .
	manualset3
256301	7	426644	16	NULL	NULL	NULL	NULL	ovum 's surface	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During exocytosis of the dense vesicles an electron dense material is released which coalesces with the surface coat of the ovum to form a thin hatching envelope which eventually lifts from the ovum 's surface .
	manualset3
256290	1	426645	16	NULL	NULL	NULL	NULL	follow-up	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During follow-up , subjects with abnormal CPS had increased risks of death ( adjusted hazard ratio ( adjHR ) 1.7 , 95 % CI 1.0-2 .8 , P = .035 ) and institutionalization ( adjHR 2.7 , 95 % CI 1.3-5 .3 , P = .006 ) , independent of demographic , health and functional status .
	manualset3
256291	2	426645	16	NULL	NULL	NULL	NULL	subjects	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During follow-up , subjects with abnormal CPS had increased risks of death ( adjusted hazard ratio ( adjHR ) 1.7 , 95 % CI 1.0-2 .8 , P = .035 ) and institutionalization ( adjHR 2.7 , 95 % CI 1.3-5 .3 , P = .006 ) , independent of demographic , health and functional status .
	manualset3
256292	3	426645	16	NULL	NULL	NULL	NULL	abnormal CPS	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During follow-up , subjects with abnormal CPS had increased risks of death ( adjusted hazard ratio ( adjHR ) 1.7 , 95 % CI 1.0-2 .8 , P = .035 ) and institutionalization ( adjHR 2.7 , 95 % CI 1.3-5 .3 , P = .006 ) , independent of demographic , health and functional status .
	manualset3
256293	4	426645	16	NULL	NULL	NULL	NULL	risks of death	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During follow-up , subjects with abnormal CPS had increased risks of death ( adjusted hazard ratio ( adjHR ) 1.7 , 95 % CI 1.0-2 .8 , P = .035 ) and institutionalization ( adjHR 2.7 , 95 % CI 1.3-5 .3 , P = .006 ) , independent of demographic , health and functional status .
	manualset3
256294	5	426645	16	NULL	NULL	NULL	NULL	adjusted hazard ratio ( adjHR )	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During follow-up , subjects with abnormal CPS had increased risks of death ( adjusted hazard ratio ( adjHR ) 1.7 , 95 % CI 1.0-2 .8 , P = .035 ) and institutionalization ( adjHR 2.7 , 95 % CI 1.3-5 .3 , P = .006 ) , independent of demographic , health and functional status .
	manualset3
256295	6	426645	16	NULL	NULL	NULL	NULL	1.7	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During follow-up , subjects with abnormal CPS had increased risks of death ( adjusted hazard ratio ( adjHR ) 1.7 , 95 % CI 1.0-2 .8 , P = .035 ) and institutionalization ( adjHR 2.7 , 95 % CI 1.3-5 .3 , P = .006 ) , independent of demographic , health and functional status .
	manualset3
256296	7	426645	16	NULL	NULL	NULL	NULL	95 % CI 1.0-2 .8	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During follow-up , subjects with abnormal CPS had increased risks of death ( adjusted hazard ratio ( adjHR ) 1.7 , 95 % CI 1.0-2 .8 , P = .035 ) and institutionalization ( adjHR 2.7 , 95 % CI 1.3-5 .3 , P = .006 ) , independent of demographic , health and functional status .
	manualset3
256297	8	426645	16	NULL	NULL	NULL	NULL	P = .035	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During follow-up , subjects with abnormal CPS had increased risks of death ( adjusted hazard ratio ( adjHR ) 1.7 , 95 % CI 1.0-2 .8 , P = .035 ) and institutionalization ( adjHR 2.7 , 95 % CI 1.3-5 .3 , P = .006 ) , independent of demographic , health and functional status .
	manualset3
256298	9	426645	16	NULL	NULL	NULL	NULL	institutionalization	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During follow-up , subjects with abnormal CPS had increased risks of death ( adjusted hazard ratio ( adjHR ) 1.7 , 95 % CI 1.0-2 .8 , P = .035 ) and institutionalization ( adjHR 2.7 , 95 % CI 1.3-5 .3 , P = .006 ) , independent of demographic , health and functional status .
	manualset3
256299	10	426645	16	NULL	NULL	NULL	NULL	adjHR 2.7	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During follow-up , subjects with abnormal CPS had increased risks of death ( adjusted hazard ratio ( adjHR ) 1.7 , 95 % CI 1.0-2 .8 , P = .035 ) and institutionalization ( adjHR 2.7 , 95 % CI 1.3-5 .3 , P = .006 ) , independent of demographic , health and functional status .
	manualset3
256300	11	426645	16	NULL	NULL	NULL	NULL	P = .006	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During follow-up , subjects with abnormal CPS had increased risks of death ( adjusted hazard ratio ( adjHR ) 1.7 , 95 % CI 1.0-2 .8 , P = .035 ) and institutionalization ( adjHR 2.7 , 95 % CI 1.3-5 .3 , P = .006 ) , independent of demographic , health and functional status .
	manualset3
256302	12	426645	16	NULL	NULL	NULL	NULL	demographic status	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During follow-up , subjects with abnormal CPS had increased risks of death ( adjusted hazard ratio ( adjHR ) 1.7 , 95 % CI 1.0-2 .8 , P = .035 ) and institutionalization ( adjHR 2.7 , 95 % CI 1.3-5 .3 , P = .006 ) , independent of demographic , health and functional status .
	manualset3
256303	13	426645	16	NULL	NULL	NULL	NULL	health status	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During follow-up , subjects with abnormal CPS had increased risks of death ( adjusted hazard ratio ( adjHR ) 1.7 , 95 % CI 1.0-2 .8 , P = .035 ) and institutionalization ( adjHR 2.7 , 95 % CI 1.3-5 .3 , P = .006 ) , independent of demographic , health and functional status .
	manualset3
256304	14	426645	16	NULL	NULL	NULL	NULL	functional status	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During follow-up , subjects with abnormal CPS had increased risks of death ( adjusted hazard ratio ( adjHR ) 1.7 , 95 % CI 1.0-2 .8 , P = .035 ) and institutionalization ( adjHR 2.7 , 95 % CI 1.3-5 .3 , P = .006 ) , independent of demographic , health and functional status .
	manualset3
256305	1	426646	16	NULL	NULL	NULL	NULL	use	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( On the use of phenatine in hypertension with asthenic syndrome in aged subjects ) .
	manualset3
256306	2	426646	16	NULL	NULL	NULL	NULL	phenatine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( On the use of phenatine in hypertension with asthenic syndrome in aged subjects ) .
	manualset3
256307	3	426646	16	NULL	NULL	NULL	NULL	hypertension	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( On the use of phenatine in hypertension with asthenic syndrome in aged subjects ) .
	manualset3
256308	4	426646	16	NULL	NULL	NULL	NULL	asthenic syndrome	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( On the use of phenatine in hypertension with asthenic syndrome in aged subjects ) .
	manualset3
256309	5	426646	16	NULL	NULL	NULL	NULL	aged subjects	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( On the use of phenatine in hypertension with asthenic syndrome in aged subjects ) .
	manualset3
256310	1	426647	16	NULL	NULL	NULL	NULL	higher river flows	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During higher river flows 90 % of the instream zinc load is attributed to diffuse sources , where inputs from resuspension of metal-rich sediments , and groundwater influx are likely to be more dominant .
	manualset3
256311	2	426647	16	NULL	NULL	NULL	NULL	90 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During higher river flows 90 % of the instream zinc load is attributed to diffuse sources , where inputs from resuspension of metal-rich sediments , and groundwater influx are likely to be more dominant .
	manualset3
256312	3	426647	16	NULL	NULL	NULL	NULL	zinc load	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During higher river flows 90 % of the instream zinc load is attributed to diffuse sources , where inputs from resuspension of metal-rich sediments , and groundwater influx are likely to be more dominant .
	manualset3
256313	4	426647	16	NULL	NULL	NULL	NULL	sources	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During higher river flows 90 % of the instream zinc load is attributed to diffuse sources , where inputs from resuspension of metal-rich sediments , and groundwater influx are likely to be more dominant .
	manualset3
256314	5	426647	16	NULL	NULL	NULL	NULL	resuspension	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During higher river flows 90 % of the instream zinc load is attributed to diffuse sources , where inputs from resuspension of metal-rich sediments , and groundwater influx are likely to be more dominant .
	manualset3
256315	6	426647	16	NULL	NULL	NULL	NULL	metal-rich sediments	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During higher river flows 90 % of the instream zinc load is attributed to diffuse sources , where inputs from resuspension of metal-rich sediments , and groundwater influx are likely to be more dominant .
	manualset3
256316	7	426647	16	NULL	NULL	NULL	NULL	influx	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During higher river flows 90 % of the instream zinc load is attributed to diffuse sources , where inputs from resuspension of metal-rich sediments , and groundwater influx are likely to be more dominant .
	manualset3
256317	1	426648	16	NULL	NULL	NULL	NULL	intravenous infusion	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During intravenous infusion of milrinone or placebo , the changes of hemodynamic parameters were monitored throughout the procedure .
	manualset3
256318	2	426648	16	NULL	NULL	NULL	NULL	milrinone	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During intravenous infusion of milrinone or placebo , the changes of hemodynamic parameters were monitored throughout the procedure .
	manualset3
256319	3	426648	16	NULL	NULL	NULL	NULL	placebo	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During intravenous infusion of milrinone or placebo , the changes of hemodynamic parameters were monitored throughout the procedure .
	manualset3
256320	4	426648	16	NULL	NULL	NULL	NULL	changes	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During intravenous infusion of milrinone or placebo , the changes of hemodynamic parameters were monitored throughout the procedure .
	manualset3
256321	5	426648	16	NULL	NULL	NULL	NULL	hemodynamic parameters	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During intravenous infusion of milrinone or placebo , the changes of hemodynamic parameters were monitored throughout the procedure .
	manualset3
256322	6	426648	16	NULL	NULL	NULL	NULL	procedure	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During intravenous infusion of milrinone or placebo , the changes of hemodynamic parameters were monitored throughout the procedure .
	manualset3
256323	1	426649	16	NULL	NULL	NULL	NULL	ischemia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During ischemia , glutamate and glycine concentrations increased several-fold when compared with baseline .
	manualset3
256324	2	426649	16	NULL	NULL	NULL	NULL	glutamate concentrations	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During ischemia , glutamate and glycine concentrations increased several-fold when compared with baseline .
	manualset3
256325	3	426649	16	NULL	NULL	NULL	NULL	glycine concentrations	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During ischemia , glutamate and glycine concentrations increased several-fold when compared with baseline .
	manualset3
256326	4	426649	16	NULL	NULL	NULL	NULL	several-fold	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During ischemia , glutamate and glycine concentrations increased several-fold when compared with baseline .
	manualset3
256327	5	426649	16	NULL	NULL	NULL	NULL	baseline	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During ischemia , glutamate and glycine concentrations increased several-fold when compared with baseline .
	manualset3
256328	1	426650	16	NULL	NULL	NULL	NULL	laparotomy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During laparotomy , the abscess was drained and the appendix was not found .
	manualset3
256329	2	426650	16	NULL	NULL	NULL	NULL	abscess	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During laparotomy , the abscess was drained and the appendix was not found .
	manualset3
256330	3	426650	16	NULL	NULL	NULL	NULL	appendix	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During laparotomy , the abscess was drained and the appendix was not found .
	manualset3
256331	1	426651	16	NULL	NULL	NULL	NULL	large-scale transitions	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During large-scale transitions from maintenance metabolic rates to maximally activated work , contrasting demands of intracellular homeostasis versus metabolic regulation obviously arise .
	manualset3
256332	2	426651	16	NULL	NULL	NULL	NULL	 maintenance metabolic rates	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During large-scale transitions from maintenance metabolic rates to maximally activated work , contrasting demands of intracellular homeostasis versus metabolic regulation obviously arise .
	manualset3
256333	3	426651	16	NULL	NULL	NULL	NULL	maximally activated work	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During large-scale transitions from maintenance metabolic rates to maximally activated work , contrasting demands of intracellular homeostasis versus metabolic regulation obviously arise .
	manualset3
256334	4	426651	16	NULL	NULL	NULL	NULL	demands	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During large-scale transitions from maintenance metabolic rates to maximally activated work , contrasting demands of intracellular homeostasis versus metabolic regulation obviously arise .
	manualset3
256335	5	426651	16	NULL	NULL	NULL	NULL	intracellular homeostasis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During large-scale transitions from maintenance metabolic rates to maximally activated work , contrasting demands of intracellular homeostasis versus metabolic regulation obviously arise .
	manualset3
256336	6	426651	16	NULL	NULL	NULL	NULL	metabolic regulation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During large-scale transitions from maintenance metabolic rates to maximally activated work , contrasting demands of intracellular homeostasis versus metabolic regulation obviously arise .
	manualset3
256337	1	426652	16	NULL	NULL	NULL	NULL	locomotion	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During locomotion of the semi-intact preparation , the discharge pattern was also very similar in homologous bilateral RS cells .
	manualset3
256338	2	426652	16	NULL	NULL	NULL	NULL	semi-intact preparation	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During locomotion of the semi-intact preparation , the discharge pattern was also very similar in homologous bilateral RS cells .
	manualset3
256339	3	426652	16	NULL	NULL	NULL	NULL	discharge pattern	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During locomotion of the semi-intact preparation , the discharge pattern was also very similar in homologous bilateral RS cells .
	manualset3
256340	4	426652	16	NULL	NULL	NULL	NULL	homologous bilateral RS cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During locomotion of the semi-intact preparation , the discharge pattern was also very similar in homologous bilateral RS cells .
	manualset3
256341	1	426653	16	NULL	NULL	NULL	NULL	long term	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During long term treatment , blood pressure was significantly decreased after felodipine during the dosing interval ( 12h ) , irrespective of concomitant treatment .
	manualset3
256342	2	426653	16	NULL	NULL	NULL	NULL	blood pressure	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During long term treatment , blood pressure was significantly decreased after felodipine during the dosing interval ( 12h ) , irrespective of concomitant treatment .
	manualset3
256343	3	426653	16	NULL	NULL	NULL	NULL	felodipine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During long term treatment , blood pressure was significantly decreased after felodipine during the dosing interval ( 12h ) , irrespective of concomitant treatment .
	manualset3
256344	4	426653	16	NULL	NULL	NULL	NULL	dosing interval	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During long term treatment , blood pressure was significantly decreased after felodipine during the dosing interval ( 12h ) , irrespective of concomitant treatment .
	manualset3
256345	5	426653	16	NULL	NULL	NULL	NULL	12h	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During long term treatment , blood pressure was significantly decreased after felodipine during the dosing interval ( 12h ) , irrespective of concomitant treatment .
	manualset3
256346	6	426653	16	NULL	NULL	NULL	NULL	treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During long term treatment , blood pressure was significantly decreased after felodipine during the dosing interval ( 12h ) , irrespective of concomitant treatment .
	manualset3
256347	1	426654	16	NULL	NULL	NULL	NULL	luteolysis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During luteolysis and for several weeks thereafter ( regressing and residual CL ) all newly formed vessels regress , which is accompanied by gradual foreshortening and rounding of endothelial cells and subsequent detachment .
	manualset3
257257	2	426654	16	NULL	NULL	NULL	NULL	several weeks	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During luteolysis and for several weeks thereafter ( regressing and residual CL ) all newly formed vessels regress , which is accompanied by gradual foreshortening and rounding of endothelial cells and subsequent detachment .
	manualset3
257259	3	426654	16	NULL	NULL	NULL	NULL	CL	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During luteolysis and for several weeks thereafter ( regressing and residual CL ) all newly formed vessels regress , which is accompanied by gradual foreshortening and rounding of endothelial cells and subsequent detachment .
	manualset3
257260	4	426654	16	NULL	NULL	NULL	NULL	vessels	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During luteolysis and for several weeks thereafter ( regressing and residual CL ) all newly formed vessels regress , which is accompanied by gradual foreshortening and rounding of endothelial cells and subsequent detachment .
	manualset3
257266	5	426654	16	NULL	NULL	NULL	NULL	rounding	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During luteolysis and for several weeks thereafter ( regressing and residual CL ) all newly formed vessels regress , which is accompanied by gradual foreshortening and rounding of endothelial cells and subsequent detachment .
	manualset3
257267	6	426654	16	NULL	NULL	NULL	NULL	endothelial cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During luteolysis and for several weeks thereafter ( regressing and residual CL ) all newly formed vessels regress , which is accompanied by gradual foreshortening and rounding of endothelial cells and subsequent detachment .
	manualset3
257271	7	426654	16	NULL	NULL	NULL	NULL	detachment	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During luteolysis and for several weeks thereafter ( regressing and residual CL ) all newly formed vessels regress , which is accompanied by gradual foreshortening and rounding of endothelial cells and subsequent detachment .
	manualset3
257275	1	426655	16	NULL	NULL	NULL	NULL	usefulness	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( On the usefulness of the so-called electro-lung for resuscitation ) .
	manualset3
257276	2	426655	16	NULL	NULL	NULL	NULL	electro-lung	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( On the usefulness of the so-called electro-lung for resuscitation ) .
	manualset3
257277	3	426655	16	NULL	NULL	NULL	NULL	resuscitation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( On the usefulness of the so-called electro-lung for resuscitation ) .
	manualset3
258007	1	426656	16	NULL	NULL	NULL	NULL	conditions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During normal conditions , intrathecal administration of MK-801 and CNQX apparently depressed mechanically and electrically ( 3 Hz ) evoked EMG responses in a dose-dependent manner ( 10 , 20 and 40 nmol in 10 microl ) .
	manualset3
258008	2	426656	16	NULL	NULL	NULL	NULL	 intrathecal administration	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During normal conditions , intrathecal administration of MK-801 and CNQX apparently depressed mechanically and electrically ( 3 Hz ) evoked EMG responses in a dose-dependent manner ( 10 , 20 and 40 nmol in 10 microl ) .
	manualset3
258009	3	426656	16	NULL	NULL	NULL	NULL	MK-801	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During normal conditions , intrathecal administration of MK-801 and CNQX apparently depressed mechanically and electrically ( 3 Hz ) evoked EMG responses in a dose-dependent manner ( 10 , 20 and 40 nmol in 10 microl ) .
	manualset3
258010	4	426656	16	NULL	NULL	NULL	NULL	CNQX	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During normal conditions , intrathecal administration of MK-801 and CNQX apparently depressed mechanically and electrically ( 3 Hz ) evoked EMG responses in a dose-dependent manner ( 10 , 20 and 40 nmol in 10 microl ) .
	manualset3
258011	5	426656	16	NULL	NULL	NULL	NULL	3 Hz	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During normal conditions , intrathecal administration of MK-801 and CNQX apparently depressed mechanically and electrically ( 3 Hz ) evoked EMG responses in a dose-dependent manner ( 10 , 20 and 40 nmol in 10 microl ) .
	manualset3
258012	6	426656	16	NULL	NULL	NULL	NULL	EMG responses	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During normal conditions , intrathecal administration of MK-801 and CNQX apparently depressed mechanically and electrically ( 3 Hz ) evoked EMG responses in a dose-dependent manner ( 10 , 20 and 40 nmol in 10 microl ) .
	manualset3
258013	7	426656	16	NULL	NULL	NULL	NULL	dose-dependent manner	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During normal conditions , intrathecal administration of MK-801 and CNQX apparently depressed mechanically and electrically ( 3 Hz ) evoked EMG responses in a dose-dependent manner ( 10 , 20 and 40 nmol in 10 microl ) .
	manualset3
258014	8	426656	16	NULL	NULL	NULL	NULL	10 nmol	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During normal conditions , intrathecal administration of MK-801 and CNQX apparently depressed mechanically and electrically ( 3 Hz ) evoked EMG responses in a dose-dependent manner ( 10 , 20 and 40 nmol in 10 microl ) .
	manualset3
258015	9	426656	16	NULL	NULL	NULL	NULL	20 nmol	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During normal conditions , intrathecal administration of MK-801 and CNQX apparently depressed mechanically and electrically ( 3 Hz ) evoked EMG responses in a dose-dependent manner ( 10 , 20 and 40 nmol in 10 microl ) .
	manualset3
258018	10	426656	16	NULL	NULL	NULL	NULL	40 nmol	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During normal conditions , intrathecal administration of MK-801 and CNQX apparently depressed mechanically and electrically ( 3 Hz ) evoked EMG responses in a dose-dependent manner ( 10 , 20 and 40 nmol in 10 microl ) .
	manualset3
258019	11	426656	16	NULL	NULL	NULL	NULL	10 microl	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During normal conditions , intrathecal administration of MK-801 and CNQX apparently depressed mechanically and electrically ( 3 Hz ) evoked EMG responses in a dose-dependent manner ( 10 , 20 and 40 nmol in 10 microl ) .
	manualset3
258020	1	426657	16	NULL	NULL	NULL	NULL	oligodendrocyte cultivation	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During oligodendrocyte cultivation we observed a significant increase in the rate of carnosine synthesis which correlates with the differentiation of these cells as revealed by immunostaining with antibodies against oligodendrocyte markers .
	manualset3
258021	2	426657	16	NULL	NULL	NULL	NULL	increase	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During oligodendrocyte cultivation we observed a significant increase in the rate of carnosine synthesis which correlates with the differentiation of these cells as revealed by immunostaining with antibodies against oligodendrocyte markers .
	manualset3
258022	3	426657	16	NULL	NULL	NULL	NULL	rate	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During oligodendrocyte cultivation we observed a significant increase in the rate of carnosine synthesis which correlates with the differentiation of these cells as revealed by immunostaining with antibodies against oligodendrocyte markers .
	manualset3
258023	4	426657	16	NULL	NULL	NULL	NULL	carnosine synthesis	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During oligodendrocyte cultivation we observed a significant increase in the rate of carnosine synthesis which correlates with the differentiation of these cells as revealed by immunostaining with antibodies against oligodendrocyte markers .
	manualset3
258024	5	426657	16	NULL	NULL	NULL	NULL	differentiation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During oligodendrocyte cultivation we observed a significant increase in the rate of carnosine synthesis which correlates with the differentiation of these cells as revealed by immunostaining with antibodies against oligodendrocyte markers .
	manualset3
258025	6	426657	16	NULL	NULL	NULL	NULL	cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During oligodendrocyte cultivation we observed a significant increase in the rate of carnosine synthesis which correlates with the differentiation of these cells as revealed by immunostaining with antibodies against oligodendrocyte markers .
	manualset3
258026	7	426657	16	NULL	NULL	NULL	NULL	immunostaining	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During oligodendrocyte cultivation we observed a significant increase in the rate of carnosine synthesis which correlates with the differentiation of these cells as revealed by immunostaining with antibodies against oligodendrocyte markers .
	manualset3
258027	8	426657	16	NULL	NULL	NULL	NULL	antibodies	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During oligodendrocyte cultivation we observed a significant increase in the rate of carnosine synthesis which correlates with the differentiation of these cells as revealed by immunostaining with antibodies against oligodendrocyte markers .
	manualset3
258028	9	426657	16	NULL	NULL	NULL	NULL	oligodendrocyte markers	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During oligodendrocyte cultivation we observed a significant increase in the rate of carnosine synthesis which correlates with the differentiation of these cells as revealed by immunostaining with antibodies against oligodendrocyte markers .
	manualset3
258029	1	426658	16	NULL	NULL	NULL	NULL	oxidation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During oxidation of succinic or other acids of the Krebs cycle , QO2 was maximal only after a long period of adaptation ( tad ) ; a latent period ( tlat ) was observed sometimes during which assimilation of oxygen was either insignificant or not detected at all .
	manualset3
258030	2	426658	16	NULL	NULL	NULL	NULL	succinic acids	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During oxidation of succinic or other acids of the Krebs cycle , QO2 was maximal only after a long period of adaptation ( tad ) ; a latent period ( tlat ) was observed sometimes during which assimilation of oxygen was either insignificant or not detected at all .
	manualset3
258254	3	426658	16	NULL	NULL	NULL	NULL	acids	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During oxidation of succinic or other acids of the Krebs cycle , QO2 was maximal only after a long period of adaptation ( tad ) ; a latent period ( tlat ) was observed sometimes during which assimilation of oxygen was either insignificant or not detected at all .
	manualset3
258255	4	426658	16	NULL	NULL	NULL	NULL	Krebs cycle	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During oxidation of succinic or other acids of the Krebs cycle , QO2 was maximal only after a long period of adaptation ( tad ) ; a latent period ( tlat ) was observed sometimes during which assimilation of oxygen was either insignificant or not detected at all .
	manualset3
258320	5	426658	16	NULL	NULL	NULL	NULL	period of adaptation ( tad )	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During oxidation of succinic or other acids of the Krebs cycle , QO2 was maximal only after a long period of adaptation ( tad ) ; a latent period ( tlat ) was observed sometimes during which assimilation of oxygen was either insignificant or not detected at all .
	manualset3
258324	6	426658	16	NULL	NULL	NULL	NULL	latent period ( tlat )	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During oxidation of succinic or other acids of the Krebs cycle , QO2 was maximal only after a long period of adaptation ( tad ) ; a latent period ( tlat ) was observed sometimes during which assimilation of oxygen was either insignificant or not detected at all .
	manualset3
258991	7	426658	16	NULL	NULL	NULL	NULL	assimilation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During oxidation of succinic or other acids of the Krebs cycle , QO2 was maximal only after a long period of adaptation ( tad ) ; a latent period ( tlat ) was observed sometimes during which assimilation of oxygen was either insignificant or not detected at all .
	manualset3
258992	8	426658	16	NULL	NULL	NULL	NULL	oxygen	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During oxidation of succinic or other acids of the Krebs cycle , QO2 was maximal only after a long period of adaptation ( tad ) ; a latent period ( tlat ) was observed sometimes during which assimilation of oxygen was either insignificant or not detected at all .
	manualset3
258993	1	426659	16	NULL	NULL	NULL	NULL	perfusion	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During perfusion of the trypsin inhibitor aprotinin an almost complete inhibition of trypsin could be observed .
	manualset3
258994	2	426659	16	NULL	NULL	NULL	NULL	trypsin inhibitor	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During perfusion of the trypsin inhibitor aprotinin an almost complete inhibition of trypsin could be observed .
	manualset3
258995	3	426659	16	NULL	NULL	NULL	NULL	aprotinin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During perfusion of the trypsin inhibitor aprotinin an almost complete inhibition of trypsin could be observed .
	manualset3
258996	4	426659	16	NULL	NULL	NULL	NULL	inhibition	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During perfusion of the trypsin inhibitor aprotinin an almost complete inhibition of trypsin could be observed .
	manualset3
258997	5	426659	16	NULL	NULL	NULL	NULL	trypsin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During perfusion of the trypsin inhibitor aprotinin an almost complete inhibition of trypsin could be observed .
	manualset3
259061	1	426660	16	NULL	NULL	NULL	NULL	preseasonal hyposensitization	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During preseasonal hyposensitization the following tendencies were found in cell sensitivity to allergen as well as in specific IgE antibody level of serum : an initial increase at the beginning of the therapy followed by a decrease during the pollen season .
	manualset3
259062	2	426660	16	NULL	NULL	NULL	NULL	tendencies	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During preseasonal hyposensitization the following tendencies were found in cell sensitivity to allergen as well as in specific IgE antibody level of serum : an initial increase at the beginning of the therapy followed by a decrease during the pollen season .
	manualset3
259063	3	426660	16	NULL	NULL	NULL	NULL	cell sensitivity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During preseasonal hyposensitization the following tendencies were found in cell sensitivity to allergen as well as in specific IgE antibody level of serum : an initial increase at the beginning of the therapy followed by a decrease during the pollen season .
	manualset3
259064	4	426660	16	NULL	NULL	NULL	NULL	allergen	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During preseasonal hyposensitization the following tendencies were found in cell sensitivity to allergen as well as in specific IgE antibody level of serum : an initial increase at the beginning of the therapy followed by a decrease during the pollen season .
	manualset3
259065	5	426660	16	NULL	NULL	NULL	NULL	serum	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During preseasonal hyposensitization the following tendencies were found in cell sensitivity to allergen as well as in specific IgE antibody level of serum : an initial increase at the beginning of the therapy followed by a decrease during the pollen season .
	manualset3
259066	6	426660	16	NULL	NULL	NULL	NULL	increase	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During preseasonal hyposensitization the following tendencies were found in cell sensitivity to allergen as well as in specific IgE antibody level of serum : an initial increase at the beginning of the therapy followed by a decrease during the pollen season .
	manualset3
259067	7	426660	16	NULL	NULL	NULL	NULL	beginning	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During preseasonal hyposensitization the following tendencies were found in cell sensitivity to allergen as well as in specific IgE antibody level of serum : an initial increase at the beginning of the therapy followed by a decrease during the pollen season .
	manualset3
259068	8	426660	16	NULL	NULL	NULL	NULL	therapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During preseasonal hyposensitization the following tendencies were found in cell sensitivity to allergen as well as in specific IgE antibody level of serum : an initial increase at the beginning of the therapy followed by a decrease during the pollen season .
	manualset3
259069	9	426660	16	NULL	NULL	NULL	NULL	decrease	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During preseasonal hyposensitization the following tendencies were found in cell sensitivity to allergen as well as in specific IgE antibody level of serum : an initial increase at the beginning of the therapy followed by a decrease during the pollen season .
	manualset3
259070	10	426660	16	NULL	NULL	NULL	NULL	pollen season	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During preseasonal hyposensitization the following tendencies were found in cell sensitivity to allergen as well as in specific IgE antibody level of serum : an initial increase at the beginning of the therapy followed by a decrease during the pollen season .
	manualset3
259071	1	426661	16	NULL	NULL	NULL	NULL	retinoic acid	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During retinoic acid-treatment , the binding of dexamethasone by intact SqCC/Y1 and CE-81T cells increased 1.5 - to 3.0-fold over 48 h. In contrast , the number of dexamethasone binding sites were decreased by 80 % in retinoic acid-treated A431 and C4-1 cells .
	manualset3
259072	2	426661	16	NULL	NULL	NULL	NULL	treatment	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During retinoic acid-treatment , the binding of dexamethasone by intact SqCC/Y1 and CE-81T cells increased 1.5 - to 3.0-fold over 48 h. In contrast , the number of dexamethasone binding sites were decreased by 80 % in retinoic acid-treated A431 and C4-1 cells .
	manualset3
259073	3	426661	16	NULL	NULL	NULL	NULL	binding	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During retinoic acid-treatment , the binding of dexamethasone by intact SqCC/Y1 and CE-81T cells increased 1.5 - to 3.0-fold over 48 h. In contrast , the number of dexamethasone binding sites were decreased by 80 % in retinoic acid-treated A431 and C4-1 cells .
	manualset3
259074	4	426661	16	NULL	NULL	NULL	NULL	dexamethasone	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During retinoic acid-treatment , the binding of dexamethasone by intact SqCC/Y1 and CE-81T cells increased 1.5 - to 3.0-fold over 48 h. In contrast , the number of dexamethasone binding sites were decreased by 80 % in retinoic acid-treated A431 and C4-1 cells .
	manualset3
259075	5	426661	16	NULL	NULL	NULL	NULL	SqCC/Y1 cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During retinoic acid-treatment , the binding of dexamethasone by intact SqCC/Y1 and CE-81T cells increased 1.5 - to 3.0-fold over 48 h. In contrast , the number of dexamethasone binding sites were decreased by 80 % in retinoic acid-treated A431 and C4-1 cells .
	manualset3
259076	6	426661	16	NULL	NULL	NULL	NULL	CE-81T cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During retinoic acid-treatment , the binding of dexamethasone by intact SqCC/Y1 and CE-81T cells increased 1.5 - to 3.0-fold over 48 h. In contrast , the number of dexamethasone binding sites were decreased by 80 % in retinoic acid-treated A431 and C4-1 cells .
	manualset3
259077	7	426661	16	NULL	NULL	NULL	NULL	1.5 - to 3.0-fold	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During retinoic acid-treatment , the binding of dexamethasone by intact SqCC/Y1 and CE-81T cells increased 1.5 - to 3.0-fold over 48 h. In contrast , the number of dexamethasone binding sites were decreased by 80 % in retinoic acid-treated A431 and C4-1 cells .
	manualset3
259078	8	426661	16	NULL	NULL	NULL	NULL	48 h	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During retinoic acid-treatment , the binding of dexamethasone by intact SqCC/Y1 and CE-81T cells increased 1.5 - to 3.0-fold over 48 h. In contrast , the number of dexamethasone binding sites were decreased by 80 % in retinoic acid-treated A431 and C4-1 cells .
	manualset3
259079	9	426661	16	NULL	NULL	NULL	NULL	contrast	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During retinoic acid-treatment , the binding of dexamethasone by intact SqCC/Y1 and CE-81T cells increased 1.5 - to 3.0-fold over 48 h. In contrast , the number of dexamethasone binding sites were decreased by 80 % in retinoic acid-treated A431 and C4-1 cells .
	manualset3
259080	10	426661	16	NULL	NULL	NULL	NULL	number	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During retinoic acid-treatment , the binding of dexamethasone by intact SqCC/Y1 and CE-81T cells increased 1.5 - to 3.0-fold over 48 h. In contrast , the number of dexamethasone binding sites were decreased by 80 % in retinoic acid-treated A431 and C4-1 cells .
	manualset3
259081	11	426661	16	NULL	NULL	NULL	NULL	dexamethasone binding sites	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During retinoic acid-treatment , the binding of dexamethasone by intact SqCC/Y1 and CE-81T cells increased 1.5 - to 3.0-fold over 48 h. In contrast , the number of dexamethasone binding sites were decreased by 80 % in retinoic acid-treated A431 and C4-1 cells .
	manualset3
259082	12	426661	16	NULL	NULL	NULL	NULL	80 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During retinoic acid-treatment , the binding of dexamethasone by intact SqCC/Y1 and CE-81T cells increased 1.5 - to 3.0-fold over 48 h. In contrast , the number of dexamethasone binding sites were decreased by 80 % in retinoic acid-treated A431 and C4-1 cells .
	manualset3
259083	13	426661	16	NULL	NULL	NULL	NULL	retinoic acid	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During retinoic acid-treatment , the binding of dexamethasone by intact SqCC/Y1 and CE-81T cells increased 1.5 - to 3.0-fold over 48 h. In contrast , the number of dexamethasone binding sites were decreased by 80 % in retinoic acid-treated A431 and C4-1 cells .
	manualset3
259084	14	426661	16	NULL	NULL	NULL	NULL	A43 cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During retinoic acid-treatment , the binding of dexamethasone by intact SqCC/Y1 and CE-81T cells increased 1.5 - to 3.0-fold over 48 h. In contrast , the number of dexamethasone binding sites were decreased by 80 % in retinoic acid-treated A431 and C4-1 cells .
	manualset3
259085	15	426661	16	NULL	NULL	NULL	NULL	C4-1 cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During retinoic acid-treatment , the binding of dexamethasone by intact SqCC/Y1 and CE-81T cells increased 1.5 - to 3.0-fold over 48 h. In contrast , the number of dexamethasone binding sites were decreased by 80 % in retinoic acid-treated A431 and C4-1 cells .
	manualset3
259086	1	426662	16	NULL	NULL	NULL	NULL	screening	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During screening of the Grx1 ( as ) genomic gene , two additional glutaredoxin pseudogenes were also isolated .
	manualset3
259087	2	426662	16	NULL	NULL	NULL	NULL	Grx1 ( as ) genomic gene	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During screening of the Grx1 ( as ) genomic gene , two additional glutaredoxin pseudogenes were also isolated .
	manualset3
259088	3	426662	16	NULL	NULL	NULL	NULL	two	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During screening of the Grx1 ( as ) genomic gene , two additional glutaredoxin pseudogenes were also isolated .
	manualset3
259089	4	426662	16	NULL	NULL	NULL	NULL	glutaredoxin pseudogenes	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During screening of the Grx1 ( as ) genomic gene , two additional glutaredoxin pseudogenes were also isolated .
	manualset3
259090	1	426663	16	NULL	NULL	NULL	NULL	self-organization	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During self-organization , nontransformed cells express morphologic and functional characteristics classically associated with the macrophage .
	manualset3
259091	2	426663	16	NULL	NULL	NULL	NULL	nontransformed cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During self-organization , nontransformed cells express morphologic and functional characteristics classically associated with the macrophage .
	manualset3
259092	3	426663	16	NULL	NULL	NULL	NULL	morphologic characteristics	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During self-organization , nontransformed cells express morphologic and functional characteristics classically associated with the macrophage .
	manualset3
259093	4	426663	16	NULL	NULL	NULL	NULL	functional characteristics	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During self-organization , nontransformed cells express morphologic and functional characteristics classically associated with the macrophage .
	manualset3
259094	5	426663	16	NULL	NULL	NULL	NULL	macrophage	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During self-organization , nontransformed cells express morphologic and functional characteristics classically associated with the macrophage .
	manualset3
259095	1	426664	16	NULL	NULL	NULL	NULL	( 14C ) Docosahexaenoic acid	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( 14C ) Docosahexaenoic acid and ( 14C ) 4 , 7 , 10 , 13 , 16-docosapentaenoic acid appeared to be less efficiently converted by the corneal enzyme than by the platelet and leukocyte enzymes .
	manualset3
259096	2	426664	16	NULL	NULL	NULL	NULL	 ( 14C ) 4 , 7 , 10 , 13 , 16-docosapentaenoic acid	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( 14C ) Docosahexaenoic acid and ( 14C ) 4 , 7 , 10 , 13 , 16-docosapentaenoic acid appeared to be less efficiently converted by the corneal enzyme than by the platelet and leukocyte enzymes .
	manualset3
259097	3	426664	16	NULL	NULL	NULL	NULL	corneal enzyme	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( 14C ) Docosahexaenoic acid and ( 14C ) 4 , 7 , 10 , 13 , 16-docosapentaenoic acid appeared to be less efficiently converted by the corneal enzyme than by the platelet and leukocyte enzymes .
	manualset3
259098	4	426664	16	NULL	NULL	NULL	NULL	platelet enzymes	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( 14C ) Docosahexaenoic acid and ( 14C ) 4 , 7 , 10 , 13 , 16-docosapentaenoic acid appeared to be less efficiently converted by the corneal enzyme than by the platelet and leukocyte enzymes .
	manualset3
259099	5	426664	16	NULL	NULL	NULL	NULL	leukocyte enzymes	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( 14C ) Docosahexaenoic acid and ( 14C ) 4 , 7 , 10 , 13 , 16-docosapentaenoic acid appeared to be less efficiently converted by the corneal enzyme than by the platelet and leukocyte enzymes .
	manualset3
259100	1	426665	16	NULL	NULL	NULL	NULL	AUTOPSY CASE	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( AUTOPSY CASE OF BRONCHIAL ASTHMA WITH DEATH DURING A SPASM ) .
	manualset3
259101	2	426665	16	NULL	NULL	NULL	NULL	BRONCHIAL ASTHMA	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( AUTOPSY CASE OF BRONCHIAL ASTHMA WITH DEATH DURING A SPASM ) .
	manualset3
259102	3	426665	16	NULL	NULL	NULL	NULL	DEATH	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( AUTOPSY CASE OF BRONCHIAL ASTHMA WITH DEATH DURING A SPASM ) .
	manualset3
259103	4	426665	16	NULL	NULL	NULL	NULL	SPASM	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( AUTOPSY CASE OF BRONCHIAL ASTHMA WITH DEATH DURING A SPASM ) .
	manualset3
259104	1	426666	16	NULL	NULL	NULL	NULL	sexual development	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During sexual development the human fungal pathogen Cryptococcus neoformans undergoes a developmental transition from yeast-form growth to filamentous growth .
	manualset3
259105	2	426666	16	NULL	NULL	NULL	NULL	fungal pathogen	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During sexual development the human fungal pathogen Cryptococcus neoformans undergoes a developmental transition from yeast-form growth to filamentous growth .
	manualset3
259106	3	426666	16	NULL	NULL	NULL	NULL	Cryptococcus neoformans	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During sexual development the human fungal pathogen Cryptococcus neoformans undergoes a developmental transition from yeast-form growth to filamentous growth .
	manualset3
259107	4	426666	16	NULL	NULL	NULL	NULL	developmental transition	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During sexual development the human fungal pathogen Cryptococcus neoformans undergoes a developmental transition from yeast-form growth to filamentous growth .
	manualset3
259108	5	426666	16	NULL	NULL	NULL	NULL	yeast-form growth	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During sexual development the human fungal pathogen Cryptococcus neoformans undergoes a developmental transition from yeast-form growth to filamentous growth .
	manualset3
259109	6	426666	16	NULL	NULL	NULL	NULL	filamentous growth	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During sexual development the human fungal pathogen Cryptococcus neoformans undergoes a developmental transition from yeast-form growth to filamentous growth .
	manualset3
259110	1	426667	16	NULL	NULL	NULL	NULL	surgical treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During surgical treatment , the uterus was replaced to its normal position followed by ovary-hysterectomy at 12h from admittance .
	manualset3
259111	2	426667	16	NULL	NULL	NULL	NULL	uterus	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During surgical treatment , the uterus was replaced to its normal position followed by ovary-hysterectomy at 12h from admittance .
	manualset3
259112	3	426667	16	NULL	NULL	NULL	NULL	normal position	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During surgical treatment , the uterus was replaced to its normal position followed by ovary-hysterectomy at 12h from admittance .
	manualset3
259113	4	426667	16	NULL	NULL	NULL	NULL	ovary-hysterectomy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During surgical treatment , the uterus was replaced to its normal position followed by ovary-hysterectomy at 12h from admittance .
	manualset3
259114	5	426667	16	NULL	NULL	NULL	NULL	12h	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During surgical treatment , the uterus was replaced to its normal position followed by ovary-hysterectomy at 12h from admittance .
	manualset3
259115	6	426667	16	NULL	NULL	NULL	NULL	admittance	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During surgical treatment , the uterus was replaced to its normal position followed by ovary-hysterectomy at 12h from admittance .
	manualset3
259162	1	426668	16	NULL	NULL	NULL	NULL	24-hour	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the 24-hour study period there was no significant difference between the two groups with respect to systemic blood pressure , mean arterial pressure , cardiac index , right atrial pressure , and pulmonary capillary wedge pressure , with the exception of a higher mean arterial pressure and systolic blood pressure at 4 hours in the albumin group and higher heart rate at 12 hours in the pentastarch group .
	manualset3
259163	2	426668	16	NULL	NULL	NULL	NULL	study period	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the 24-hour study period there was no significant difference between the two groups with respect to systemic blood pressure , mean arterial pressure , cardiac index , right atrial pressure , and pulmonary capillary wedge pressure , with the exception of a higher mean arterial pressure and systolic blood pressure at 4 hours in the albumin group and higher heart rate at 12 hours in the pentastarch group .
	manualset3
259164	3	426668	16	NULL	NULL	NULL	NULL	difference	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the 24-hour study period there was no significant difference between the two groups with respect to systemic blood pressure , mean arterial pressure , cardiac index , right atrial pressure , and pulmonary capillary wedge pressure , with the exception of a higher mean arterial pressure and systolic blood pressure at 4 hours in the albumin group and higher heart rate at 12 hours in the pentastarch group .
	manualset3
259165	4	426668	16	NULL	NULL	NULL	NULL	two	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the 24-hour study period there was no significant difference between the two groups with respect to systemic blood pressure , mean arterial pressure , cardiac index , right atrial pressure , and pulmonary capillary wedge pressure , with the exception of a higher mean arterial pressure and systolic blood pressure at 4 hours in the albumin group and higher heart rate at 12 hours in the pentastarch group .
	manualset3
259166	5	426668	16	NULL	NULL	NULL	NULL	groups	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the 24-hour study period there was no significant difference between the two groups with respect to systemic blood pressure , mean arterial pressure , cardiac index , right atrial pressure , and pulmonary capillary wedge pressure , with the exception of a higher mean arterial pressure and systolic blood pressure at 4 hours in the albumin group and higher heart rate at 12 hours in the pentastarch group .
	manualset3
259167	6	426668	16	NULL	NULL	NULL	NULL	systemic blood pressure	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the 24-hour study period there was no significant difference between the two groups with respect to systemic blood pressure , mean arterial pressure , cardiac index , right atrial pressure , and pulmonary capillary wedge pressure , with the exception of a higher mean arterial pressure and systolic blood pressure at 4 hours in the albumin group and higher heart rate at 12 hours in the pentastarch group .
	manualset3
259170	7	426668	16	NULL	NULL	NULL	NULL	mean arterial pressure	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the 24-hour study period there was no significant difference between the two groups with respect to systemic blood pressure , mean arterial pressure , cardiac index , right atrial pressure , and pulmonary capillary wedge pressure , with the exception of a higher mean arterial pressure and systolic blood pressure at 4 hours in the albumin group and higher heart rate at 12 hours in the pentastarch group .
	manualset3
259172	8	426668	16	NULL	NULL	NULL	NULL	cardiac index	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the 24-hour study period there was no significant difference between the two groups with respect to systemic blood pressure , mean arterial pressure , cardiac index , right atrial pressure , and pulmonary capillary wedge pressure , with the exception of a higher mean arterial pressure and systolic blood pressure at 4 hours in the albumin group and higher heart rate at 12 hours in the pentastarch group .
	manualset3
259175	9	426668	16	NULL	NULL	NULL	NULL	right atrial pressure	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the 24-hour study period there was no significant difference between the two groups with respect to systemic blood pressure , mean arterial pressure , cardiac index , right atrial pressure , and pulmonary capillary wedge pressure , with the exception of a higher mean arterial pressure and systolic blood pressure at 4 hours in the albumin group and higher heart rate at 12 hours in the pentastarch group .
	manualset3
259176	10	426668	16	NULL	NULL	NULL	NULL	pulmonary capillary wedge pressure	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the 24-hour study period there was no significant difference between the two groups with respect to systemic blood pressure , mean arterial pressure , cardiac index , right atrial pressure , and pulmonary capillary wedge pressure , with the exception of a higher mean arterial pressure and systolic blood pressure at 4 hours in the albumin group and higher heart rate at 12 hours in the pentastarch group .
	manualset3
259177	11	426668	16	NULL	NULL	NULL	NULL	mean arterial pressure	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the 24-hour study period there was no significant difference between the two groups with respect to systemic blood pressure , mean arterial pressure , cardiac index , right atrial pressure , and pulmonary capillary wedge pressure , with the exception of a higher mean arterial pressure and systolic blood pressure at 4 hours in the albumin group and higher heart rate at 12 hours in the pentastarch group .
	manualset3
259178	12	426668	16	NULL	NULL	NULL	NULL	systolic blood pressure	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the 24-hour study period there was no significant difference between the two groups with respect to systemic blood pressure , mean arterial pressure , cardiac index , right atrial pressure , and pulmonary capillary wedge pressure , with the exception of a higher mean arterial pressure and systolic blood pressure at 4 hours in the albumin group and higher heart rate at 12 hours in the pentastarch group .
	manualset3
259179	13	426668	16	NULL	NULL	NULL	NULL	4 hours	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the 24-hour study period there was no significant difference between the two groups with respect to systemic blood pressure , mean arterial pressure , cardiac index , right atrial pressure , and pulmonary capillary wedge pressure , with the exception of a higher mean arterial pressure and systolic blood pressure at 4 hours in the albumin group and higher heart rate at 12 hours in the pentastarch group .
	manualset3
259180	14	426668	16	NULL	NULL	NULL	NULL	albumin group	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the 24-hour study period there was no significant difference between the two groups with respect to systemic blood pressure , mean arterial pressure , cardiac index , right atrial pressure , and pulmonary capillary wedge pressure , with the exception of a higher mean arterial pressure and systolic blood pressure at 4 hours in the albumin group and higher heart rate at 12 hours in the pentastarch group .
	manualset3
259183	15	426668	16	NULL	NULL	NULL	NULL	heart rate	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the 24-hour study period there was no significant difference between the two groups with respect to systemic blood pressure , mean arterial pressure , cardiac index , right atrial pressure , and pulmonary capillary wedge pressure , with the exception of a higher mean arterial pressure and systolic blood pressure at 4 hours in the albumin group and higher heart rate at 12 hours in the pentastarch group .
	manualset3
259185	16	426668	16	NULL	NULL	NULL	NULL	12 hours	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the 24-hour study period there was no significant difference between the two groups with respect to systemic blood pressure , mean arterial pressure , cardiac index , right atrial pressure , and pulmonary capillary wedge pressure , with the exception of a higher mean arterial pressure and systolic blood pressure at 4 hours in the albumin group and higher heart rate at 12 hours in the pentastarch group .
	manualset3
259186	17	426668	16	NULL	NULL	NULL	NULL	pentastarch group	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the 24-hour study period there was no significant difference between the two groups with respect to systemic blood pressure , mean arterial pressure , cardiac index , right atrial pressure , and pulmonary capillary wedge pressure , with the exception of a higher mean arterial pressure and systolic blood pressure at 4 hours in the albumin group and higher heart rate at 12 hours in the pentastarch group .
	manualset3
259336	1	426669	16	NULL	NULL	NULL	NULL	8 days	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the 8 days of the study , an average of 48.3 % of the ETU ingested in wine was excreted unmodified by the kidneys .
	manualset3
259337	2	426669	16	NULL	NULL	NULL	NULL	study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the 8 days of the study , an average of 48.3 % of the ETU ingested in wine was excreted unmodified by the kidneys .
	manualset3
259338	3	426669	16	NULL	NULL	NULL	NULL	average	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the 8 days of the study , an average of 48.3 % of the ETU ingested in wine was excreted unmodified by the kidneys .
	manualset3
259339	4	426669	16	NULL	NULL	NULL	NULL	48.3 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the 8 days of the study , an average of 48.3 % of the ETU ingested in wine was excreted unmodified by the kidneys .
	manualset3
259340	5	426669	16	NULL	NULL	NULL	NULL	ETU	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the 8 days of the study , an average of 48.3 % of the ETU ingested in wine was excreted unmodified by the kidneys .
	manualset3
259341	6	426669	16	NULL	NULL	NULL	NULL	wine	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the 8 days of the study , an average of 48.3 % of the ETU ingested in wine was excreted unmodified by the kidneys .
	manualset3
259342	7	426669	16	NULL	NULL	NULL	NULL	kidneys	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the 8 days of the study , an average of 48.3 % of the ETU ingested in wine was excreted unmodified by the kidneys .
	manualset3
259343	1	426670	16	NULL	NULL	NULL	NULL	active deposition	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the active deposition of calcium phosphate , however , a new , higher molecular weight form of pyrophosphatase activity was produced suggesting that this enzyme activity is associated with biological mineralization .
	manualset3
259344	2	426670	16	NULL	NULL	NULL	NULL	calcium phosphate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the active deposition of calcium phosphate , however , a new , higher molecular weight form of pyrophosphatase activity was produced suggesting that this enzyme activity is associated with biological mineralization .
	manualset3
259345	3	426670	16	NULL	NULL	NULL	NULL	higher molecular weight form	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the active deposition of calcium phosphate , however , a new , higher molecular weight form of pyrophosphatase activity was produced suggesting that this enzyme activity is associated with biological mineralization .
	manualset3
259346	4	426670	16	NULL	NULL	NULL	NULL	pyrophosphatase activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the active deposition of calcium phosphate , however , a new , higher molecular weight form of pyrophosphatase activity was produced suggesting that this enzyme activity is associated with biological mineralization .
	manualset3
259347	5	426670	16	NULL	NULL	NULL	NULL	enzyme activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the active deposition of calcium phosphate , however , a new , higher molecular weight form of pyrophosphatase activity was produced suggesting that this enzyme activity is associated with biological mineralization .
	manualset3
259348	6	426670	16	NULL	NULL	NULL	NULL	 biological mineralization	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the active deposition of calcium phosphate , however , a new , higher molecular weight form of pyrophosphatase activity was produced suggesting that this enzyme activity is associated with biological mineralization .
	manualset3
259349	1	426671	16	NULL	NULL	NULL	NULL	active period	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the active period of the East Asia monsoon and the Indian summer monsoon , stable isotopes in precipitation events had significant negative correlations with south wind index ( r = - 0.354 for deltaD and r = - 0.390 for delta18O , p & lt ; 0.05 , respectively ) , indicating that isotopic values closely associated with the origin and transport of moisture , and especially the Indian summer monsoon could bring vapors with very low isotopic values and d-excess values .
	manualset3
259350	2	426671	16	NULL	NULL	NULL	NULL	East Asia monsoon	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the active period of the East Asia monsoon and the Indian summer monsoon , stable isotopes in precipitation events had significant negative correlations with south wind index ( r = - 0.354 for deltaD and r = - 0.390 for delta18O , p & lt ; 0.05 , respectively ) , indicating that isotopic values closely associated with the origin and transport of moisture , and especially the Indian summer monsoon could bring vapors with very low isotopic values and d-excess values .
	manualset3
259351	3	426671	16	NULL	NULL	NULL	NULL	Indian summer monsoon	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the active period of the East Asia monsoon and the Indian summer monsoon , stable isotopes in precipitation events had significant negative correlations with south wind index ( r = - 0.354 for deltaD and r = - 0.390 for delta18O , p & lt ; 0.05 , respectively ) , indicating that isotopic values closely associated with the origin and transport of moisture , and especially the Indian summer monsoon could bring vapors with very low isotopic values and d-excess values .
	manualset3
259352	4	426671	16	NULL	NULL	NULL	NULL	stable isotopes	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the active period of the East Asia monsoon and the Indian summer monsoon , stable isotopes in precipitation events had significant negative correlations with south wind index ( r = - 0.354 for deltaD and r = - 0.390 for delta18O , p & lt ; 0.05 , respectively ) , indicating that isotopic values closely associated with the origin and transport of moisture , and especially the Indian summer monsoon could bring vapors with very low isotopic values and d-excess values .
	manualset3
259353	5	426671	16	NULL	NULL	NULL	NULL	precipitation events	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the active period of the East Asia monsoon and the Indian summer monsoon , stable isotopes in precipitation events had significant negative correlations with south wind index ( r = - 0.354 for deltaD and r = - 0.390 for delta18O , p & lt ; 0.05 , respectively ) , indicating that isotopic values closely associated with the origin and transport of moisture , and especially the Indian summer monsoon could bring vapors with very low isotopic values and d-excess values .
	manualset3
259354	6	426671	16	NULL	NULL	NULL	NULL	negative correlations	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the active period of the East Asia monsoon and the Indian summer monsoon , stable isotopes in precipitation events had significant negative correlations with south wind index ( r = - 0.354 for deltaD and r = - 0.390 for delta18O , p & lt ; 0.05 , respectively ) , indicating that isotopic values closely associated with the origin and transport of moisture , and especially the Indian summer monsoon could bring vapors with very low isotopic values and d-excess values .
	manualset3
259355	7	426671	16	NULL	NULL	NULL	NULL	south wind index	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the active period of the East Asia monsoon and the Indian summer monsoon , stable isotopes in precipitation events had significant negative correlations with south wind index ( r = - 0.354 for deltaD and r = - 0.390 for delta18O , p & lt ; 0.05 , respectively ) , indicating that isotopic values closely associated with the origin and transport of moisture , and especially the Indian summer monsoon could bring vapors with very low isotopic values and d-excess values .
	manualset3
259356	8	426671	16	NULL	NULL	NULL	NULL	 r = - 0.354 for deltaD	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the active period of the East Asia monsoon and the Indian summer monsoon , stable isotopes in precipitation events had significant negative correlations with south wind index ( r = - 0.354 for deltaD and r = - 0.390 for delta18O , p & lt ; 0.05 , respectively ) , indicating that isotopic values closely associated with the origin and transport of moisture , and especially the Indian summer monsoon could bring vapors with very low isotopic values and d-excess values .
	manualset3
259357	9	426671	16	NULL	NULL	NULL	NULL	r = - 0.390 for delta18O	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the active period of the East Asia monsoon and the Indian summer monsoon , stable isotopes in precipitation events had significant negative correlations with south wind index ( r = - 0.354 for deltaD and r = - 0.390 for delta18O , p & lt ; 0.05 , respectively ) , indicating that isotopic values closely associated with the origin and transport of moisture , and especially the Indian summer monsoon could bring vapors with very low isotopic values and d-excess values .
	manualset3
259358	10	426671	16	NULL	NULL	NULL	NULL	 p & lt ; 0.05	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the active period of the East Asia monsoon and the Indian summer monsoon , stable isotopes in precipitation events had significant negative correlations with south wind index ( r = - 0.354 for deltaD and r = - 0.390 for delta18O , p & lt ; 0.05 , respectively ) , indicating that isotopic values closely associated with the origin and transport of moisture , and especially the Indian summer monsoon could bring vapors with very low isotopic values and d-excess values .
	manualset3
259359	11	426671	16	NULL	NULL	NULL	NULL	isotopic values	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the active period of the East Asia monsoon and the Indian summer monsoon , stable isotopes in precipitation events had significant negative correlations with south wind index ( r = - 0.354 for deltaD and r = - 0.390 for delta18O , p & lt ; 0.05 , respectively ) , indicating that isotopic values closely associated with the origin and transport of moisture , and especially the Indian summer monsoon could bring vapors with very low isotopic values and d-excess values .
	manualset3
259360	12	426671	16	NULL	NULL	NULL	NULL	origin	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the active period of the East Asia monsoon and the Indian summer monsoon , stable isotopes in precipitation events had significant negative correlations with south wind index ( r = - 0.354 for deltaD and r = - 0.390 for delta18O , p & lt ; 0.05 , respectively ) , indicating that isotopic values closely associated with the origin and transport of moisture , and especially the Indian summer monsoon could bring vapors with very low isotopic values and d-excess values .
	manualset3
259361	13	426671	16	NULL	NULL	NULL	NULL	transport	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the active period of the East Asia monsoon and the Indian summer monsoon , stable isotopes in precipitation events had significant negative correlations with south wind index ( r = - 0.354 for deltaD and r = - 0.390 for delta18O , p & lt ; 0.05 , respectively ) , indicating that isotopic values closely associated with the origin and transport of moisture , and especially the Indian summer monsoon could bring vapors with very low isotopic values and d-excess values .
	manualset3
259362	14	426671	16	NULL	NULL	NULL	NULL	moisture	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the active period of the East Asia monsoon and the Indian summer monsoon , stable isotopes in precipitation events had significant negative correlations with south wind index ( r = - 0.354 for deltaD and r = - 0.390 for delta18O , p & lt ; 0.05 , respectively ) , indicating that isotopic values closely associated with the origin and transport of moisture , and especially the Indian summer monsoon could bring vapors with very low isotopic values and d-excess values .
	manualset3
259363	15	426671	16	NULL	NULL	NULL	NULL	 Indian summer monsoon	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the active period of the East Asia monsoon and the Indian summer monsoon , stable isotopes in precipitation events had significant negative correlations with south wind index ( r = - 0.354 for deltaD and r = - 0.390 for delta18O , p & lt ; 0.05 , respectively ) , indicating that isotopic values closely associated with the origin and transport of moisture , and especially the Indian summer monsoon could bring vapors with very low isotopic values and d-excess values .
	manualset3
259364	16	426671	16	NULL	NULL	NULL	NULL	vapors	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the active period of the East Asia monsoon and the Indian summer monsoon , stable isotopes in precipitation events had significant negative correlations with south wind index ( r = - 0.354 for deltaD and r = - 0.390 for delta18O , p & lt ; 0.05 , respectively ) , indicating that isotopic values closely associated with the origin and transport of moisture , and especially the Indian summer monsoon could bring vapors with very low isotopic values and d-excess values .
	manualset3
259365	17	426671	16	NULL	NULL	NULL	NULL	isotopic values	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the active period of the East Asia monsoon and the Indian summer monsoon , stable isotopes in precipitation events had significant negative correlations with south wind index ( r = - 0.354 for deltaD and r = - 0.390 for delta18O , p & lt ; 0.05 , respectively ) , indicating that isotopic values closely associated with the origin and transport of moisture , and especially the Indian summer monsoon could bring vapors with very low isotopic values and d-excess values .
	manualset3
259366	18	426671	16	NULL	NULL	NULL	NULL	d-excess values	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the active period of the East Asia monsoon and the Indian summer monsoon , stable isotopes in precipitation events had significant negative correlations with south wind index ( r = - 0.354 for deltaD and r = - 0.390 for delta18O , p & lt ; 0.05 , respectively ) , indicating that isotopic values closely associated with the origin and transport of moisture , and especially the Indian summer monsoon could bring vapors with very low isotopic values and d-excess values .
	manualset3
259367	1	426672	16	NULL	NULL	NULL	NULL	application	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the application of IOEM general anesthesia should be provided by total intravenous anesthesia with propofol with an emphasis on a continuous high opioid dosage .
	manualset3
259368	2	426672	16	NULL	NULL	NULL	NULL	 IOEM general anesthesia	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the application of IOEM general anesthesia should be provided by total intravenous anesthesia with propofol with an emphasis on a continuous high opioid dosage .
	manualset3
259369	3	426672	16	NULL	NULL	NULL	NULL	total intravenous anesthesia	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the application of IOEM general anesthesia should be provided by total intravenous anesthesia with propofol with an emphasis on a continuous high opioid dosage .
	manualset3
259370	4	426672	16	NULL	NULL	NULL	NULL	propofol	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the application of IOEM general anesthesia should be provided by total intravenous anesthesia with propofol with an emphasis on a continuous high opioid dosage .
	manualset3
259371	5	426672	16	NULL	NULL	NULL	NULL	emphasis	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the application of IOEM general anesthesia should be provided by total intravenous anesthesia with propofol with an emphasis on a continuous high opioid dosage .
	manualset3
259372	6	426672	16	NULL	NULL	NULL	NULL	opioid	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the application of IOEM general anesthesia should be provided by total intravenous anesthesia with propofol with an emphasis on a continuous high opioid dosage .
	manualset3
259373	7	426672	16	NULL	NULL	NULL	NULL	dosage	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the application of IOEM general anesthesia should be provided by total intravenous anesthesia with propofol with an emphasis on a continuous high opioid dosage .
	manualset3
259374	1	426673	16	NULL	NULL	NULL	NULL	diagnostic workup	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the diagnostic workup , the patient experienced fever due to hospital based pneumonia , which unmasked typical ST segment changes of Brugada syndrome .
	manualset3
259375	2	426673	16	NULL	NULL	NULL	NULL	patient	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the diagnostic workup , the patient experienced fever due to hospital based pneumonia , which unmasked typical ST segment changes of Brugada syndrome .
	manualset3
259376	3	426673	16	NULL	NULL	NULL	NULL	fever	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the diagnostic workup , the patient experienced fever due to hospital based pneumonia , which unmasked typical ST segment changes of Brugada syndrome .
	manualset3
259377	4	426673	16	NULL	NULL	NULL	NULL	hospital based pneumonia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the diagnostic workup , the patient experienced fever due to hospital based pneumonia , which unmasked typical ST segment changes of Brugada syndrome .
	manualset3
259378	5	426673	16	NULL	NULL	NULL	NULL	ST segment changes	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the diagnostic workup , the patient experienced fever due to hospital based pneumonia , which unmasked typical ST segment changes of Brugada syndrome .
	manualset3
259379	6	426673	16	NULL	NULL	NULL	NULL	Brugada syndrome	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the diagnostic workup , the patient experienced fever due to hospital based pneumonia , which unmasked typical ST segment changes of Brugada syndrome .
	manualset3
259380	1	426674	16	NULL	NULL	NULL	NULL	Open pelvic fracture	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Open pelvic fracture -- an indication for laparotomy ? ) .
	manualset3
259381	2	426674	16	NULL	NULL	NULL	NULL	indication	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Open pelvic fracture -- an indication for laparotomy ? ) .
	manualset3
259382	3	426674	16	NULL	NULL	NULL	NULL	laparotomy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Open pelvic fracture -- an indication for laparotomy ? ) .
	manualset3
259383	1	426675	16	NULL	NULL	NULL	NULL	expulsion	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the expulsion of foetuses , NEFA and cortisol levels increased ( +18 and +30 % , respectively ) , and they decreased immediately after the birth of the last piglet , to reach the initial levels observed before farrowing ( around 700 microEq.L-1 and 110 ng.mL-1 , respectively ) .
	manualset3
259384	2	426675	16	NULL	NULL	NULL	NULL	foetuses	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the expulsion of foetuses , NEFA and cortisol levels increased ( +18 and +30 % , respectively ) , and they decreased immediately after the birth of the last piglet , to reach the initial levels observed before farrowing ( around 700 microEq.L-1 and 110 ng.mL-1 , respectively ) .
	manualset3
259385	3	426675	16	NULL	NULL	NULL	NULL	NEFA	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the expulsion of foetuses , NEFA and cortisol levels increased ( +18 and +30 % , respectively ) , and they decreased immediately after the birth of the last piglet , to reach the initial levels observed before farrowing ( around 700 microEq.L-1 and 110 ng.mL-1 , respectively ) .
	manualset3
259386	4	426675	16	NULL	NULL	NULL	NULL	cortisol levels	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the expulsion of foetuses , NEFA and cortisol levels increased ( +18 and +30 % , respectively ) , and they decreased immediately after the birth of the last piglet , to reach the initial levels observed before farrowing ( around 700 microEq.L-1 and 110 ng.mL-1 , respectively ) .
	manualset3
259387	5	426675	16	NULL	NULL	NULL	NULL	+18 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the expulsion of foetuses , NEFA and cortisol levels increased ( +18 and +30 % , respectively ) , and they decreased immediately after the birth of the last piglet , to reach the initial levels observed before farrowing ( around 700 microEq.L-1 and 110 ng.mL-1 , respectively ) .
	manualset3
259388	6	426675	16	NULL	NULL	NULL	NULL	+30 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the expulsion of foetuses , NEFA and cortisol levels increased ( +18 and +30 % , respectively ) , and they decreased immediately after the birth of the last piglet , to reach the initial levels observed before farrowing ( around 700 microEq.L-1 and 110 ng.mL-1 , respectively ) .
	manualset3
259389	7	426675	16	NULL	NULL	NULL	NULL	birth	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the expulsion of foetuses , NEFA and cortisol levels increased ( +18 and +30 % , respectively ) , and they decreased immediately after the birth of the last piglet , to reach the initial levels observed before farrowing ( around 700 microEq.L-1 and 110 ng.mL-1 , respectively ) .
	manualset3
259390	8	426675	16	NULL	NULL	NULL	NULL	last	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the expulsion of foetuses , NEFA and cortisol levels increased ( +18 and +30 % , respectively ) , and they decreased immediately after the birth of the last piglet , to reach the initial levels observed before farrowing ( around 700 microEq.L-1 and 110 ng.mL-1 , respectively ) .
	manualset3
259391	9	426675	16	NULL	NULL	NULL	NULL	piglet	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the expulsion of foetuses , NEFA and cortisol levels increased ( +18 and +30 % , respectively ) , and they decreased immediately after the birth of the last piglet , to reach the initial levels observed before farrowing ( around 700 microEq.L-1 and 110 ng.mL-1 , respectively ) .
	manualset3
259392	10	426675	16	NULL	NULL	NULL	NULL	initial levels	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the expulsion of foetuses , NEFA and cortisol levels increased ( +18 and +30 % , respectively ) , and they decreased immediately after the birth of the last piglet , to reach the initial levels observed before farrowing ( around 700 microEq.L-1 and 110 ng.mL-1 , respectively ) .
	manualset3
259393	11	426675	16	NULL	NULL	NULL	NULL	farrowing	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the expulsion of foetuses , NEFA and cortisol levels increased ( +18 and +30 % , respectively ) , and they decreased immediately after the birth of the last piglet , to reach the initial levels observed before farrowing ( around 700 microEq.L-1 and 110 ng.mL-1 , respectively ) .
	manualset3
259394	12	426675	16	NULL	NULL	NULL	NULL	700 microEq.L-1	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the expulsion of foetuses , NEFA and cortisol levels increased ( +18 and +30 % , respectively ) , and they decreased immediately after the birth of the last piglet , to reach the initial levels observed before farrowing ( around 700 microEq.L-1 and 110 ng.mL-1 , respectively ) .
	manualset3
259395	13	426675	16	NULL	NULL	NULL	NULL	110 ng.mL-1	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the expulsion of foetuses , NEFA and cortisol levels increased ( +18 and +30 % , respectively ) , and they decreased immediately after the birth of the last piglet , to reach the initial levels observed before farrowing ( around 700 microEq.L-1 and 110 ng.mL-1 , respectively ) .
	manualset3
259396	1	426676	16	NULL	NULL	NULL	NULL	first 24 h	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the first 24 h of GnRH therapy there was a small increase in immunoreactive ( 5.4 + / - 0.8 IU/l ) and bioactive ( 6.7 + / - 1.3 IU/l ) LH , with an irregular pattern and little effect on testosterone production ( 2.2 nmol/l ) .
	manualset3
259397	2	426676	16	NULL	NULL	NULL	NULL	GnRH therapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the first 24 h of GnRH therapy there was a small increase in immunoreactive ( 5.4 + / - 0.8 IU/l ) and bioactive ( 6.7 + / - 1.3 IU/l ) LH , with an irregular pattern and little effect on testosterone production ( 2.2 nmol/l ) .
	manualset3
259398	3	426676	16	NULL	NULL	NULL	NULL	increase	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the first 24 h of GnRH therapy there was a small increase in immunoreactive ( 5.4 + / - 0.8 IU/l ) and bioactive ( 6.7 + / - 1.3 IU/l ) LH , with an irregular pattern and little effect on testosterone production ( 2.2 nmol/l ) .
	manualset3
259399	4	426676	16	NULL	NULL	NULL	NULL	immunoreactive LH	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the first 24 h of GnRH therapy there was a small increase in immunoreactive ( 5.4 + / - 0.8 IU/l ) and bioactive ( 6.7 + / - 1.3 IU/l ) LH , with an irregular pattern and little effect on testosterone production ( 2.2 nmol/l ) .
	manualset3
259400	5	426676	16	NULL	NULL	NULL	NULL	5.4 + / - 0.8 IU/l	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the first 24 h of GnRH therapy there was a small increase in immunoreactive ( 5.4 + / - 0.8 IU/l ) and bioactive ( 6.7 + / - 1.3 IU/l ) LH , with an irregular pattern and little effect on testosterone production ( 2.2 nmol/l ) .
	manualset3
259401	6	426676	16	NULL	NULL	NULL	NULL	bioactive LH	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the first 24 h of GnRH therapy there was a small increase in immunoreactive ( 5.4 + / - 0.8 IU/l ) and bioactive ( 6.7 + / - 1.3 IU/l ) LH , with an irregular pattern and little effect on testosterone production ( 2.2 nmol/l ) .
	manualset3
259402	7	426676	16	NULL	NULL	NULL	NULL	6.7 + / - 1.3 IU/l	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the first 24 h of GnRH therapy there was a small increase in immunoreactive ( 5.4 + / - 0.8 IU/l ) and bioactive ( 6.7 + / - 1.3 IU/l ) LH , with an irregular pattern and little effect on testosterone production ( 2.2 nmol/l ) .
	manualset3
259403	8	426676	16	NULL	NULL	NULL	NULL	irregular pattern	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the first 24 h of GnRH therapy there was a small increase in immunoreactive ( 5.4 + / - 0.8 IU/l ) and bioactive ( 6.7 + / - 1.3 IU/l ) LH , with an irregular pattern and little effect on testosterone production ( 2.2 nmol/l ) .
	manualset3
259404	9	426676	16	NULL	NULL	NULL	NULL	effect	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the first 24 h of GnRH therapy there was a small increase in immunoreactive ( 5.4 + / - 0.8 IU/l ) and bioactive ( 6.7 + / - 1.3 IU/l ) LH , with an irregular pattern and little effect on testosterone production ( 2.2 nmol/l ) .
	manualset3
259405	10	426676	16	NULL	NULL	NULL	NULL	testosterone production	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the first 24 h of GnRH therapy there was a small increase in immunoreactive ( 5.4 + / - 0.8 IU/l ) and bioactive ( 6.7 + / - 1.3 IU/l ) LH , with an irregular pattern and little effect on testosterone production ( 2.2 nmol/l ) .
	manualset3
259406	11	426676	16	NULL	NULL	NULL	NULL	2.2 nmol/l	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the first 24 h of GnRH therapy there was a small increase in immunoreactive ( 5.4 + / - 0.8 IU/l ) and bioactive ( 6.7 + / - 1.3 IU/l ) LH , with an irregular pattern and little effect on testosterone production ( 2.2 nmol/l ) .
	manualset3
259519	1	426677	16	NULL	NULL	NULL	NULL	first month	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the first month of treatment , adolescents who reported increased life crisis events experienced greater symptom severity following naproxen therapy .
	manualset3
259520	2	426677	16	NULL	NULL	NULL	NULL	treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the first month of treatment , adolescents who reported increased life crisis events experienced greater symptom severity following naproxen therapy .
	manualset3
259521	3	426677	16	NULL	NULL	NULL	NULL	adolescents	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the first month of treatment , adolescents who reported increased life crisis events experienced greater symptom severity following naproxen therapy .
	manualset3
259522	4	426677	16	NULL	NULL	NULL	NULL	life crisis events	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the first month of treatment , adolescents who reported increased life crisis events experienced greater symptom severity following naproxen therapy .
	manualset3
260005	5	426677	16	NULL	NULL	NULL	NULL	symptom severity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the first month of treatment , adolescents who reported increased life crisis events experienced greater symptom severity following naproxen therapy .
	manualset3
260007	6	426677	16	NULL	NULL	NULL	NULL	naproxen	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the first month of treatment , adolescents who reported increased life crisis events experienced greater symptom severity following naproxen therapy .
	manualset3
260008	7	426677	16	NULL	NULL	NULL	NULL	therapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the first month of treatment , adolescents who reported increased life crisis events experienced greater symptom severity following naproxen therapy .
	manualset3
260013	1	426678	16	NULL	NULL	NULL	NULL	growth period	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the growth period of summer maize , the NO3 - - N content in leached water in fertilization treatments had two peaks , while the NH4 + - N content had a trend of increased first and decreased then .
	manualset3
260015	2	426678	16	NULL	NULL	NULL	NULL	summer maize	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the growth period of summer maize , the NO3 - - N content in leached water in fertilization treatments had two peaks , while the NH4 + - N content had a trend of increased first and decreased then .
	manualset3
260020	3	426678	16	NULL	NULL	NULL	NULL	NO3 - - N content	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the growth period of summer maize , the NO3 - - N content in leached water in fertilization treatments had two peaks , while the NH4 + - N content had a trend of increased first and decreased then .
	manualset3
260022	4	426678	16	NULL	NULL	NULL	NULL	leached water	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the growth period of summer maize , the NO3 - - N content in leached water in fertilization treatments had two peaks , while the NH4 + - N content had a trend of increased first and decreased then .
	manualset3
260032	5	426678	16	NULL	NULL	NULL	NULL	fertilization treatments	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the growth period of summer maize , the NO3 - - N content in leached water in fertilization treatments had two peaks , while the NH4 + - N content had a trend of increased first and decreased then .
	manualset3
260033	6	426678	16	NULL	NULL	NULL	NULL	two peaks	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the growth period of summer maize , the NO3 - - N content in leached water in fertilization treatments had two peaks , while the NH4 + - N content had a trend of increased first and decreased then .
	manualset3
260034	7	426678	16	NULL	NULL	NULL	NULL	NH4 + - N content	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the growth period of summer maize , the NO3 - - N content in leached water in fertilization treatments had two peaks , while the NH4 + - N content had a trend of increased first and decreased then .
	manualset3
260035	8	426678	16	NULL	NULL	NULL	NULL	trend	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the growth period of summer maize , the NO3 - - N content in leached water in fertilization treatments had two peaks , while the NH4 + - N content had a trend of increased first and decreased then .
	manualset3
260036	9	426678	16	NULL	NULL	NULL	NULL	first	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the growth period of summer maize , the NO3 - - N content in leached water in fertilization treatments had two peaks , while the NH4 + - N content had a trend of increased first and decreased then .
	manualset3
260141	1	426679	16	NULL	NULL	NULL	NULL	initial stage	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the initial stage of neuromuscular junction ( NMJ ) formation , nerve-derived agrin cooperates with muscle-autonomous mechanisms in the organization and stabilization of a plaque-like postsynaptic specialization at the site of nerve-muscle contact .
	manualset3
260143	2	426679	16	NULL	NULL	NULL	NULL	neuromuscular junction ( NMJ ) formation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the initial stage of neuromuscular junction ( NMJ ) formation , nerve-derived agrin cooperates with muscle-autonomous mechanisms in the organization and stabilization of a plaque-like postsynaptic specialization at the site of nerve-muscle contact .
	manualset3
260144	3	426679	16	NULL	NULL	NULL	NULL	nerve-derived agrin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the initial stage of neuromuscular junction ( NMJ ) formation , nerve-derived agrin cooperates with muscle-autonomous mechanisms in the organization and stabilization of a plaque-like postsynaptic specialization at the site of nerve-muscle contact .
	manualset3
260145	4	426679	16	NULL	NULL	NULL	NULL	muscle-autonomous mechanisms	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the initial stage of neuromuscular junction ( NMJ ) formation , nerve-derived agrin cooperates with muscle-autonomous mechanisms in the organization and stabilization of a plaque-like postsynaptic specialization at the site of nerve-muscle contact .
	manualset3
260146	5	426679	16	NULL	NULL	NULL	NULL	organization	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the initial stage of neuromuscular junction ( NMJ ) formation , nerve-derived agrin cooperates with muscle-autonomous mechanisms in the organization and stabilization of a plaque-like postsynaptic specialization at the site of nerve-muscle contact .
	manualset3
260147	6	426679	16	NULL	NULL	NULL	NULL	stabilization	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the initial stage of neuromuscular junction ( NMJ ) formation , nerve-derived agrin cooperates with muscle-autonomous mechanisms in the organization and stabilization of a plaque-like postsynaptic specialization at the site of nerve-muscle contact .
	manualset3
260148	7	426679	16	NULL	NULL	NULL	NULL	plaque-like postsynaptic specialization	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the initial stage of neuromuscular junction ( NMJ ) formation , nerve-derived agrin cooperates with muscle-autonomous mechanisms in the organization and stabilization of a plaque-like postsynaptic specialization at the site of nerve-muscle contact .
	manualset3
260149	8	426679	16	NULL	NULL	NULL	NULL	site	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the initial stage of neuromuscular junction ( NMJ ) formation , nerve-derived agrin cooperates with muscle-autonomous mechanisms in the organization and stabilization of a plaque-like postsynaptic specialization at the site of nerve-muscle contact .
	manualset3
260150	9	426679	16	NULL	NULL	NULL	NULL	nerve-muscle contact	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the initial stage of neuromuscular junction ( NMJ ) formation , nerve-derived agrin cooperates with muscle-autonomous mechanisms in the organization and stabilization of a plaque-like postsynaptic specialization at the site of nerve-muscle contact .
	manualset3
260151	1	426680	16	NULL	NULL	NULL	NULL	initial stages	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the initial stages of cardiac stimulation or defibrillation , the distribution of transmembrane potential generated in the myocardium by the external stimulus is determined by the local interactions between fibrous tissue organization and applied electric field .
	manualset3
260152	2	426680	16	NULL	NULL	NULL	NULL	cardiac stimulation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the initial stages of cardiac stimulation or defibrillation , the distribution of transmembrane potential generated in the myocardium by the external stimulus is determined by the local interactions between fibrous tissue organization and applied electric field .
	manualset3
260153	3	426680	16	NULL	NULL	NULL	NULL	defibrillation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the initial stages of cardiac stimulation or defibrillation , the distribution of transmembrane potential generated in the myocardium by the external stimulus is determined by the local interactions between fibrous tissue organization and applied electric field .
	manualset3
260154	4	426680	16	NULL	NULL	NULL	NULL	distribution	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the initial stages of cardiac stimulation or defibrillation , the distribution of transmembrane potential generated in the myocardium by the external stimulus is determined by the local interactions between fibrous tissue organization and applied electric field .
	manualset3
260155	5	426680	16	NULL	NULL	NULL	NULL	transmembrane potential	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the initial stages of cardiac stimulation or defibrillation , the distribution of transmembrane potential generated in the myocardium by the external stimulus is determined by the local interactions between fibrous tissue organization and applied electric field .
	manualset3
260156	6	426680	16	NULL	NULL	NULL	NULL	myocardium	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the initial stages of cardiac stimulation or defibrillation , the distribution of transmembrane potential generated in the myocardium by the external stimulus is determined by the local interactions between fibrous tissue organization and applied electric field .
	manualset3
260157	7	426680	16	NULL	NULL	NULL	NULL	external stimulus	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the initial stages of cardiac stimulation or defibrillation , the distribution of transmembrane potential generated in the myocardium by the external stimulus is determined by the local interactions between fibrous tissue organization and applied electric field .
	manualset3
260158	8	426680	16	NULL	NULL	NULL	NULL	local interactions	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the initial stages of cardiac stimulation or defibrillation , the distribution of transmembrane potential generated in the myocardium by the external stimulus is determined by the local interactions between fibrous tissue organization and applied electric field .
	manualset3
262119	9	426680	16	NULL	NULL	NULL	NULL	fibrous tissue organization	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the initial stages of cardiac stimulation or defibrillation , the distribution of transmembrane potential generated in the myocardium by the external stimulus is determined by the local interactions between fibrous tissue organization and applied electric field .
	manualset3
262120	10	426680	16	NULL	NULL	NULL	NULL	applied electric field	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the initial stages of cardiac stimulation or defibrillation , the distribution of transmembrane potential generated in the myocardium by the external stimulus is determined by the local interactions between fibrous tissue organization and applied electric field .
	manualset3
262121	1	426681	16	NULL	NULL	NULL	NULL	Ophthalmoplegic migraine	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Ophthalmoplegic migraine with alternating ophthalmoplegia and exophthalmos ) .
	manualset3
262122	2	426681	16	NULL	NULL	NULL	NULL	ophthalmoplegia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Ophthalmoplegic migraine with alternating ophthalmoplegia and exophthalmos ) .
	manualset3
262123	3	426681	16	NULL	NULL	NULL	NULL	exophthalmos	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Ophthalmoplegic migraine with alternating ophthalmoplegia and exophthalmos ) .
	manualset3
262124	1	426682	16	NULL	NULL	NULL	NULL	last decade	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the last decade , involvement of growth hormone ( GH ) , insulin-like growth factors ( IGFs ) and IGF binding proteins ( IGFBPs ) in ovarian folliculogenesis has been extensively studied .
	manualset3
262125	2	426682	16	NULL	NULL	NULL	NULL	involvement	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the last decade , involvement of growth hormone ( GH ) , insulin-like growth factors ( IGFs ) and IGF binding proteins ( IGFBPs ) in ovarian folliculogenesis has been extensively studied .
	manualset3
262126	3	426682	16	NULL	NULL	NULL	NULL	growth hormone ( GH )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the last decade , involvement of growth hormone ( GH ) , insulin-like growth factors ( IGFs ) and IGF binding proteins ( IGFBPs ) in ovarian folliculogenesis has been extensively studied .
	manualset3
262127	4	426682	16	NULL	NULL	NULL	NULL	insulin-like growth factors ( IGFs )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the last decade , involvement of growth hormone ( GH ) , insulin-like growth factors ( IGFs ) and IGF binding proteins ( IGFBPs ) in ovarian folliculogenesis has been extensively studied .
	manualset3
262128	5	426682	16	NULL	NULL	NULL	NULL	IGF binding proteins ( IGFBPs )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the last decade , involvement of growth hormone ( GH ) , insulin-like growth factors ( IGFs ) and IGF binding proteins ( IGFBPs ) in ovarian folliculogenesis has been extensively studied .
	manualset3
262129	6	426682	16	NULL	NULL	NULL	NULL	ovarian folliculogenesis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the last decade , involvement of growth hormone ( GH ) , insulin-like growth factors ( IGFs ) and IGF binding proteins ( IGFBPs ) in ovarian folliculogenesis has been extensively studied .
	manualset3
262130	1	426683	16	NULL	NULL	NULL	NULL	last decade	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the last decade laparoscopy has been proposed as a less invasive approach when surgery is indicated .
	manualset3
262131	2	426683	16	NULL	NULL	NULL	NULL	laparoscopy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the last decade laparoscopy has been proposed as a less invasive approach when surgery is indicated .
	manualset3
262132	3	426683	16	NULL	NULL	NULL	NULL	less invasive approach	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the last decade laparoscopy has been proposed as a less invasive approach when surgery is indicated .
	manualset3
262133	4	426683	16	NULL	NULL	NULL	NULL	surgery	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the last decade laparoscopy has been proposed as a less invasive approach when surgery is indicated .
	manualset3
262167	1	426684	16	NULL	NULL	NULL	NULL	last five years	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the last five years , various structures were described with a high selectivity for D4 receptor subtype .
	manualset3
262169	2	426684	16	NULL	NULL	NULL	NULL	structures	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the last five years , various structures were described with a high selectivity for D4 receptor subtype .
	manualset3
262170	3	426684	16	NULL	NULL	NULL	NULL	high selectivity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the last five years , various structures were described with a high selectivity for D4 receptor subtype .
	manualset3
262173	4	426684	16	NULL	NULL	NULL	NULL	D4 receptor subtype	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the last five years , various structures were described with a high selectivity for D4 receptor subtype .
	manualset3
262174	1	426685	16	NULL	NULL	NULL	NULL	last two decades	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the last two decades an increasing amount of information has been accumulated regarding the gene structure and organization of the mitochondrial genome from various organisms .
	manualset3
262175	2	426685	16	NULL	NULL	NULL	NULL	amount	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the last two decades an increasing amount of information has been accumulated regarding the gene structure and organization of the mitochondrial genome from various organisms .
	manualset3
262176	3	426685	16	NULL	NULL	NULL	NULL	information	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the last two decades an increasing amount of information has been accumulated regarding the gene structure and organization of the mitochondrial genome from various organisms .
	manualset3
262177	4	426685	16	NULL	NULL	NULL	NULL	gene structure	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the last two decades an increasing amount of information has been accumulated regarding the gene structure and organization of the mitochondrial genome from various organisms .
	manualset3
262178	5	426685	16	NULL	NULL	NULL	NULL	organization	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the last two decades an increasing amount of information has been accumulated regarding the gene structure and organization of the mitochondrial genome from various organisms .
	manualset3
262179	6	426685	16	NULL	NULL	NULL	NULL	mitochondrial genome	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the last two decades an increasing amount of information has been accumulated regarding the gene structure and organization of the mitochondrial genome from various organisms .
	manualset3
262180	7	426685	16	NULL	NULL	NULL	NULL	organisms	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the last two decades an increasing amount of information has been accumulated regarding the gene structure and organization of the mitochondrial genome from various organisms .
	manualset3
262181	1	426686	16	NULL	NULL	NULL	NULL	late epidemic period	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the late epidemic period , a strain that failed to ferment sucrose dominated cholera outbreaks in the Northern Brazilian Amazon region .
	manualset3
262182	2	426686	16	NULL	NULL	NULL	NULL	strain	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the late epidemic period , a strain that failed to ferment sucrose dominated cholera outbreaks in the Northern Brazilian Amazon region .
	manualset3
262183	3	426686	16	NULL	NULL	NULL	NULL	sucrose	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the late epidemic period , a strain that failed to ferment sucrose dominated cholera outbreaks in the Northern Brazilian Amazon region .
	manualset3
262184	4	426686	16	NULL	NULL	NULL	NULL	cholera outbreaks	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the late epidemic period , a strain that failed to ferment sucrose dominated cholera outbreaks in the Northern Brazilian Amazon region .
	manualset3
262185	5	426686	16	NULL	NULL	NULL	NULL	Northern Brazilian Amazon region	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the late epidemic period , a strain that failed to ferment sucrose dominated cholera outbreaks in the Northern Brazilian Amazon region .
	manualset3
262186	1	426687	16	NULL	NULL	NULL	NULL	lifestyle modification	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the lifestyle modification , there was a significant decrease in body weight among obese teenagers , associated with an increase in ghrelin ( apparent from month 6 ; P & lt ; 0.05 ) , a decrease in leptin ( from month 3 ; P & lt ; 0.05 ) and a decrease in insulin and HOMA ( from month 3 ; P & lt ; 0.0001 ) , without any significant change in PYY .
	manualset3
262187	2	426687	16	NULL	NULL	NULL	NULL	significant decrease	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the lifestyle modification , there was a significant decrease in body weight among obese teenagers , associated with an increase in ghrelin ( apparent from month 6 ; P & lt ; 0.05 ) , a decrease in leptin ( from month 3 ; P & lt ; 0.05 ) and a decrease in insulin and HOMA ( from month 3 ; P & lt ; 0.0001 ) , without any significant change in PYY .
	manualset3
262188	3	426687	16	NULL	NULL	NULL	NULL	body weight	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the lifestyle modification , there was a significant decrease in body weight among obese teenagers , associated with an increase in ghrelin ( apparent from month 6 ; P & lt ; 0.05 ) , a decrease in leptin ( from month 3 ; P & lt ; 0.05 ) and a decrease in insulin and HOMA ( from month 3 ; P & lt ; 0.0001 ) , without any significant change in PYY .
	manualset3
262189	4	426687	16	NULL	NULL	NULL	NULL	obese teenagers	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the lifestyle modification , there was a significant decrease in body weight among obese teenagers , associated with an increase in ghrelin ( apparent from month 6 ; P & lt ; 0.05 ) , a decrease in leptin ( from month 3 ; P & lt ; 0.05 ) and a decrease in insulin and HOMA ( from month 3 ; P & lt ; 0.0001 ) , without any significant change in PYY .
	manualset3
262251	5	426687	16	NULL	NULL	NULL	NULL	increase	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the lifestyle modification , there was a significant decrease in body weight among obese teenagers , associated with an increase in ghrelin ( apparent from month 6 ; P & lt ; 0.05 ) , a decrease in leptin ( from month 3 ; P & lt ; 0.05 ) and a decrease in insulin and HOMA ( from month 3 ; P & lt ; 0.0001 ) , without any significant change in PYY .
	manualset3
262252	6	426687	16	NULL	NULL	NULL	NULL	ghrelin	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the lifestyle modification , there was a significant decrease in body weight among obese teenagers , associated with an increase in ghrelin ( apparent from month 6 ; P & lt ; 0.05 ) , a decrease in leptin ( from month 3 ; P & lt ; 0.05 ) and a decrease in insulin and HOMA ( from month 3 ; P & lt ; 0.0001 ) , without any significant change in PYY .
	manualset3
262497	7	426687	16	NULL	NULL	NULL	NULL	month 6	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the lifestyle modification , there was a significant decrease in body weight among obese teenagers , associated with an increase in ghrelin ( apparent from month 6 ; P & lt ; 0.05 ) , a decrease in leptin ( from month 3 ; P & lt ; 0.05 ) and a decrease in insulin and HOMA ( from month 3 ; P & lt ; 0.0001 ) , without any significant change in PYY .
	manualset3
262499	8	426687	16	NULL	NULL	NULL	NULL	P & lt ; 0.05	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the lifestyle modification , there was a significant decrease in body weight among obese teenagers , associated with an increase in ghrelin ( apparent from month 6 ; P & lt ; 0.05 ) , a decrease in leptin ( from month 3 ; P & lt ; 0.05 ) and a decrease in insulin and HOMA ( from month 3 ; P & lt ; 0.0001 ) , without any significant change in PYY .
	manualset3
262501	9	426687	16	NULL	NULL	NULL	NULL	decrease	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the lifestyle modification , there was a significant decrease in body weight among obese teenagers , associated with an increase in ghrelin ( apparent from month 6 ; P & lt ; 0.05 ) , a decrease in leptin ( from month 3 ; P & lt ; 0.05 ) and a decrease in insulin and HOMA ( from month 3 ; P & lt ; 0.0001 ) , without any significant change in PYY .
	manualset3
262504	10	426687	16	NULL	NULL	NULL	NULL	leptin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the lifestyle modification , there was a significant decrease in body weight among obese teenagers , associated with an increase in ghrelin ( apparent from month 6 ; P & lt ; 0.05 ) , a decrease in leptin ( from month 3 ; P & lt ; 0.05 ) and a decrease in insulin and HOMA ( from month 3 ; P & lt ; 0.0001 ) , without any significant change in PYY .
	manualset3
262505	11	426687	16	NULL	NULL	NULL	NULL	month 3	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the lifestyle modification , there was a significant decrease in body weight among obese teenagers , associated with an increase in ghrelin ( apparent from month 6 ; P & lt ; 0.05 ) , a decrease in leptin ( from month 3 ; P & lt ; 0.05 ) and a decrease in insulin and HOMA ( from month 3 ; P & lt ; 0.0001 ) , without any significant change in PYY .
	manualset3
262508	12	426687	16	NULL	NULL	NULL	NULL	P & lt ; 0.05	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the lifestyle modification , there was a significant decrease in body weight among obese teenagers , associated with an increase in ghrelin ( apparent from month 6 ; P & lt ; 0.05 ) , a decrease in leptin ( from month 3 ; P & lt ; 0.05 ) and a decrease in insulin and HOMA ( from month 3 ; P & lt ; 0.0001 ) , without any significant change in PYY .
	manualset3
262511	13	426687	16	NULL	NULL	NULL	NULL	decrease	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the lifestyle modification , there was a significant decrease in body weight among obese teenagers , associated with an increase in ghrelin ( apparent from month 6 ; P & lt ; 0.05 ) , a decrease in leptin ( from month 3 ; P & lt ; 0.05 ) and a decrease in insulin and HOMA ( from month 3 ; P & lt ; 0.0001 ) , without any significant change in PYY .
	manualset3
262516	14	426687	16	NULL	NULL	NULL	NULL	insulin	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the lifestyle modification , there was a significant decrease in body weight among obese teenagers , associated with an increase in ghrelin ( apparent from month 6 ; P & lt ; 0.05 ) , a decrease in leptin ( from month 3 ; P & lt ; 0.05 ) and a decrease in insulin and HOMA ( from month 3 ; P & lt ; 0.0001 ) , without any significant change in PYY .
	manualset3
262529	15	426687	16	NULL	NULL	NULL	NULL	HOMA	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the lifestyle modification , there was a significant decrease in body weight among obese teenagers , associated with an increase in ghrelin ( apparent from month 6 ; P & lt ; 0.05 ) , a decrease in leptin ( from month 3 ; P & lt ; 0.05 ) and a decrease in insulin and HOMA ( from month 3 ; P & lt ; 0.0001 ) , without any significant change in PYY .
	manualset3
262532	16	426687	16	NULL	NULL	NULL	NULL	month 3	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the lifestyle modification , there was a significant decrease in body weight among obese teenagers , associated with an increase in ghrelin ( apparent from month 6 ; P & lt ; 0.05 ) , a decrease in leptin ( from month 3 ; P & lt ; 0.05 ) and a decrease in insulin and HOMA ( from month 3 ; P & lt ; 0.0001 ) , without any significant change in PYY .
	manualset3
262534	17	426687	16	NULL	NULL	NULL	NULL	P & lt ; 0.0001	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the lifestyle modification , there was a significant decrease in body weight among obese teenagers , associated with an increase in ghrelin ( apparent from month 6 ; P & lt ; 0.05 ) , a decrease in leptin ( from month 3 ; P & lt ; 0.05 ) and a decrease in insulin and HOMA ( from month 3 ; P & lt ; 0.0001 ) , without any significant change in PYY .
	manualset3
262539	18	426687	16	NULL	NULL	NULL	NULL	change	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the lifestyle modification , there was a significant decrease in body weight among obese teenagers , associated with an increase in ghrelin ( apparent from month 6 ; P & lt ; 0.05 ) , a decrease in leptin ( from month 3 ; P & lt ; 0.05 ) and a decrease in insulin and HOMA ( from month 3 ; P & lt ; 0.0001 ) , without any significant change in PYY .
	manualset3
262540	19	426687	16	NULL	NULL	NULL	NULL	PYY	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the lifestyle modification , there was a significant decrease in body weight among obese teenagers , associated with an increase in ghrelin ( apparent from month 6 ; P & lt ; 0.05 ) , a decrease in leptin ( from month 3 ; P & lt ; 0.05 ) and a decrease in insulin and HOMA ( from month 3 ; P & lt ; 0.0001 ) , without any significant change in PYY .
	manualset3
262559	1	426688	16	NULL	NULL	NULL	NULL	low illumination	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the low illumination only ( EZ ) - and ( ZE ) - bilirubin and ( EZ ) - cyclobilirubin appeared in the urine ; during the high illumination ( EE ) - bilirubin and ( EE ) - cyclobilirubin also appeared , showing a similar excretion pattern to that observed in the bile , but the total urinary excretion rates were lower than the total biliary excretion rates .
	manualset3
262573	2	426688	16	NULL	NULL	NULL	NULL	( EZ ) -  bilirubin	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the low illumination only ( EZ ) - and ( ZE ) - bilirubin and ( EZ ) - cyclobilirubin appeared in the urine ; during the high illumination ( EE ) - bilirubin and ( EE ) - cyclobilirubin also appeared , showing a similar excretion pattern to that observed in the bile , but the total urinary excretion rates were lower than the total biliary excretion rates .
	manualset3
262575	3	426688	16	NULL	NULL	NULL	NULL	( ZE ) - bilirubin	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the low illumination only ( EZ ) - and ( ZE ) - bilirubin and ( EZ ) - cyclobilirubin appeared in the urine ; during the high illumination ( EE ) - bilirubin and ( EE ) - cyclobilirubin also appeared , showing a similar excretion pattern to that observed in the bile , but the total urinary excretion rates were lower than the total biliary excretion rates .
	manualset3
262576	4	426688	16	NULL	NULL	NULL	NULL	( EZ ) - cyclobilirubin	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the low illumination only ( EZ ) - and ( ZE ) - bilirubin and ( EZ ) - cyclobilirubin appeared in the urine ; during the high illumination ( EE ) - bilirubin and ( EE ) - cyclobilirubin also appeared , showing a similar excretion pattern to that observed in the bile , but the total urinary excretion rates were lower than the total biliary excretion rates .
	manualset3
263355	5	426688	16	NULL	NULL	NULL	NULL	urine	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the low illumination only ( EZ ) - and ( ZE ) - bilirubin and ( EZ ) - cyclobilirubin appeared in the urine ; during the high illumination ( EE ) - bilirubin and ( EE ) - cyclobilirubin also appeared , showing a similar excretion pattern to that observed in the bile , but the total urinary excretion rates were lower than the total biliary excretion rates .
	manualset3
263356	6	426688	16	NULL	NULL	NULL	NULL	high illumination	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the low illumination only ( EZ ) - and ( ZE ) - bilirubin and ( EZ ) - cyclobilirubin appeared in the urine ; during the high illumination ( EE ) - bilirubin and ( EE ) - cyclobilirubin also appeared , showing a similar excretion pattern to that observed in the bile , but the total urinary excretion rates were lower than the total biliary excretion rates .
	manualset3
263357	7	426688	16	NULL	NULL	NULL	NULL	( EE ) - bilirubin	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the low illumination only ( EZ ) - and ( ZE ) - bilirubin and ( EZ ) - cyclobilirubin appeared in the urine ; during the high illumination ( EE ) - bilirubin and ( EE ) - cyclobilirubin also appeared , showing a similar excretion pattern to that observed in the bile , but the total urinary excretion rates were lower than the total biliary excretion rates .
	manualset3
263358	8	426688	16	NULL	NULL	NULL	NULL	( EE ) - cyclobilirubin	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the low illumination only ( EZ ) - and ( ZE ) - bilirubin and ( EZ ) - cyclobilirubin appeared in the urine ; during the high illumination ( EE ) - bilirubin and ( EE ) - cyclobilirubin also appeared , showing a similar excretion pattern to that observed in the bile , but the total urinary excretion rates were lower than the total biliary excretion rates .
	manualset3
263359	9	426688	16	NULL	NULL	NULL	NULL	excretion pattern	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the low illumination only ( EZ ) - and ( ZE ) - bilirubin and ( EZ ) - cyclobilirubin appeared in the urine ; during the high illumination ( EE ) - bilirubin and ( EE ) - cyclobilirubin also appeared , showing a similar excretion pattern to that observed in the bile , but the total urinary excretion rates were lower than the total biliary excretion rates .
	manualset3
263360	10	426688	16	NULL	NULL	NULL	NULL	bile	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the low illumination only ( EZ ) - and ( ZE ) - bilirubin and ( EZ ) - cyclobilirubin appeared in the urine ; during the high illumination ( EE ) - bilirubin and ( EE ) - cyclobilirubin also appeared , showing a similar excretion pattern to that observed in the bile , but the total urinary excretion rates were lower than the total biliary excretion rates .
	manualset3
263361	11	426688	16	NULL	NULL	NULL	NULL	 total urinary excretion rates	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the low illumination only ( EZ ) - and ( ZE ) - bilirubin and ( EZ ) - cyclobilirubin appeared in the urine ; during the high illumination ( EE ) - bilirubin and ( EE ) - cyclobilirubin also appeared , showing a similar excretion pattern to that observed in the bile , but the total urinary excretion rates were lower than the total biliary excretion rates .
	manualset3
263362	12	426688	16	NULL	NULL	NULL	NULL	total biliary excretion rates	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the low illumination only ( EZ ) - and ( ZE ) - bilirubin and ( EZ ) - cyclobilirubin appeared in the urine ; during the high illumination ( EE ) - bilirubin and ( EE ) - cyclobilirubin also appeared , showing a similar excretion pattern to that observed in the bile , but the total urinary excretion rates were lower than the total biliary excretion rates .
	manualset3
263363	1	426689	16	NULL	NULL	NULL	NULL	nonischemic control periods	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the nonischemic control periods , the peak rise in coronary vascular resistance with acetylstrophanthidin was 16 + / -1 % above control ( P less than 0.01 ) .
	manualset3
263364	2	426689	16	NULL	NULL	NULL	NULL	peak rise	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the nonischemic control periods , the peak rise in coronary vascular resistance with acetylstrophanthidin was 16 + / -1 % above control ( P less than 0.01 ) .
	manualset3
263365	3	426689	16	NULL	NULL	NULL	NULL	coronary vascular resistance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the nonischemic control periods , the peak rise in coronary vascular resistance with acetylstrophanthidin was 16 + / -1 % above control ( P less than 0.01 ) .
	manualset3
263366	4	426689	16	NULL	NULL	NULL	NULL	acetylstrophanthidin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the nonischemic control periods , the peak rise in coronary vascular resistance with acetylstrophanthidin was 16 + / -1 % above control ( P less than 0.01 ) .
	manualset3
263367	5	426689	16	NULL	NULL	NULL	NULL	16 + / -1 %	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the nonischemic control periods , the peak rise in coronary vascular resistance with acetylstrophanthidin was 16 + / -1 % above control ( P less than 0.01 ) .
	manualset3
263368	6	426689	16	NULL	NULL	NULL	NULL	control	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the nonischemic control periods , the peak rise in coronary vascular resistance with acetylstrophanthidin was 16 + / -1 % above control ( P less than 0.01 ) .
	manualset3
263369	7	426689	16	NULL	NULL	NULL	NULL	P less than 0.01	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the nonischemic control periods , the peak rise in coronary vascular resistance with acetylstrophanthidin was 16 + / -1 % above control ( P less than 0.01 ) .
	manualset3
263370	1	426690	16	NULL	NULL	NULL	NULL	past six years	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the past six years , great progress has been made in defining the key cellular and molecular signalling pathways that determine the fate of cardiac myocytes after ischaemia-reperfusion ( IR ) and consequently the severity of myocardial infarction .
	manualset3
263371	2	426690	16	NULL	NULL	NULL	NULL	progress	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the past six years , great progress has been made in defining the key cellular and molecular signalling pathways that determine the fate of cardiac myocytes after ischaemia-reperfusion ( IR ) and consequently the severity of myocardial infarction .
	manualset3
263372	3	426690	16	NULL	NULL	NULL	NULL	cellular signalling pathways	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the past six years , great progress has been made in defining the key cellular and molecular signalling pathways that determine the fate of cardiac myocytes after ischaemia-reperfusion ( IR ) and consequently the severity of myocardial infarction .
	manualset3
263373	4	426690	16	NULL	NULL	NULL	NULL	molecular signalling pathways	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the past six years , great progress has been made in defining the key cellular and molecular signalling pathways that determine the fate of cardiac myocytes after ischaemia-reperfusion ( IR ) and consequently the severity of myocardial infarction .
	manualset3
263374	5	426690	16	NULL	NULL	NULL	NULL	fate	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the past six years , great progress has been made in defining the key cellular and molecular signalling pathways that determine the fate of cardiac myocytes after ischaemia-reperfusion ( IR ) and consequently the severity of myocardial infarction .
	manualset3
263375	6	426690	16	NULL	NULL	NULL	NULL	cardiac myocytes	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the past six years , great progress has been made in defining the key cellular and molecular signalling pathways that determine the fate of cardiac myocytes after ischaemia-reperfusion ( IR ) and consequently the severity of myocardial infarction .
	manualset3
263376	7	426690	16	NULL	NULL	NULL	NULL	ischaemia-reperfusion ( IR )	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the past six years , great progress has been made in defining the key cellular and molecular signalling pathways that determine the fate of cardiac myocytes after ischaemia-reperfusion ( IR ) and consequently the severity of myocardial infarction .
	manualset3
263377	8	426690	16	NULL	NULL	NULL	NULL	severity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the past six years , great progress has been made in defining the key cellular and molecular signalling pathways that determine the fate of cardiac myocytes after ischaemia-reperfusion ( IR ) and consequently the severity of myocardial infarction .
	manualset3
263378	9	426690	16	NULL	NULL	NULL	NULL	myocardial infarction	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the past six years , great progress has been made in defining the key cellular and molecular signalling pathways that determine the fate of cardiac myocytes after ischaemia-reperfusion ( IR ) and consequently the severity of myocardial infarction .
	manualset3
263379	1	426691	16	NULL	NULL	NULL	NULL	patent period	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the patent period , mice fed alpha whey fraction had significantly higher blood total white cell , CD4 + and CD8 + lymphocyte counts and higher Con A-stimulated IFN-gamma production by spleen cells than those fed other protein sources , but there was no significant difference in output of faecal oocysts .
	manualset3
263380	2	426691	16	NULL	NULL	NULL	NULL	mice	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the patent period , mice fed alpha whey fraction had significantly higher blood total white cell , CD4 + and CD8 + lymphocyte counts and higher Con A-stimulated IFN-gamma production by spleen cells than those fed other protein sources , but there was no significant difference in output of faecal oocysts .
	manualset3
263381	3	426691	16	NULL	NULL	NULL	NULL	alpha whey fraction	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the patent period , mice fed alpha whey fraction had significantly higher blood total white cell , CD4 + and CD8 + lymphocyte counts and higher Con A-stimulated IFN-gamma production by spleen cells than those fed other protein sources , but there was no significant difference in output of faecal oocysts .
	manualset3
263382	4	426691	16	NULL	NULL	NULL	NULL	blood total white cell	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the patent period , mice fed alpha whey fraction had significantly higher blood total white cell , CD4 + and CD8 + lymphocyte counts and higher Con A-stimulated IFN-gamma production by spleen cells than those fed other protein sources , but there was no significant difference in output of faecal oocysts .
	manualset3
263383	5	426691	16	NULL	NULL	NULL	NULL	CD4 + lymphocyte counts	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the patent period , mice fed alpha whey fraction had significantly higher blood total white cell , CD4 + and CD8 + lymphocyte counts and higher Con A-stimulated IFN-gamma production by spleen cells than those fed other protein sources , but there was no significant difference in output of faecal oocysts .
	manualset3
263384	6	426691	16	NULL	NULL	NULL	NULL	CD8 + lymphocyte counts	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the patent period , mice fed alpha whey fraction had significantly higher blood total white cell , CD4 + and CD8 + lymphocyte counts and higher Con A-stimulated IFN-gamma production by spleen cells than those fed other protein sources , but there was no significant difference in output of faecal oocysts .
	manualset3
263385	7	426691	16	NULL	NULL	NULL	NULL	Con A-stimulated IFN-gamma production	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the patent period , mice fed alpha whey fraction had significantly higher blood total white cell , CD4 + and CD8 + lymphocyte counts and higher Con A-stimulated IFN-gamma production by spleen cells than those fed other protein sources , but there was no significant difference in output of faecal oocysts .
	manualset3
263386	8	426691	16	NULL	NULL	NULL	NULL	spleen cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the patent period , mice fed alpha whey fraction had significantly higher blood total white cell , CD4 + and CD8 + lymphocyte counts and higher Con A-stimulated IFN-gamma production by spleen cells than those fed other protein sources , but there was no significant difference in output of faecal oocysts .
	manualset3
263387	9	426691	16	NULL	NULL	NULL	NULL	protein sources	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the patent period , mice fed alpha whey fraction had significantly higher blood total white cell , CD4 + and CD8 + lymphocyte counts and higher Con A-stimulated IFN-gamma production by spleen cells than those fed other protein sources , but there was no significant difference in output of faecal oocysts .
	manualset3
263388	10	426691	16	NULL	NULL	NULL	NULL	output	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the patent period , mice fed alpha whey fraction had significantly higher blood total white cell , CD4 + and CD8 + lymphocyte counts and higher Con A-stimulated IFN-gamma production by spleen cells than those fed other protein sources , but there was no significant difference in output of faecal oocysts .
	manualset3
263389	11	426691	16	NULL	NULL	NULL	NULL	faecal oocysts	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the patent period , mice fed alpha whey fraction had significantly higher blood total white cell , CD4 + and CD8 + lymphocyte counts and higher Con A-stimulated IFN-gamma production by spleen cells than those fed other protein sources , but there was no significant difference in output of faecal oocysts .
	manualset3
263390	1	426692	16	NULL	NULL	NULL	NULL	research and development process	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the research and development process many similar chemicals or materials may be synthesized that accomplish the required task .
	manualset3
263391	2	426692	16	NULL	NULL	NULL	NULL	chemicals	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the research and development process many similar chemicals or materials may be synthesized that accomplish the required task .
	manualset3
263392	3	426692	16	NULL	NULL	NULL	NULL	materials	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the research and development process many similar chemicals or materials may be synthesized that accomplish the required task .
	manualset3
263393	4	426692	16	NULL	NULL	NULL	NULL	task	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the research and development process many similar chemicals or materials may be synthesized that accomplish the required task .
	manualset3
263394	1	426693	16	NULL	NULL	NULL	NULL	running process	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the running process , CB ( 7 ) bears a positive charge in the pH range of 2.5-7 .5 and can be adsorbed onto the inner wall of a fused-capillary , leading to a reversal of the electroosmotic flow ( EOF ) .
	manualset3
263395	2	426693	16	NULL	NULL	NULL	NULL	CB ( 7 )	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the running process , CB ( 7 ) bears a positive charge in the pH range of 2.5-7 .5 and can be adsorbed onto the inner wall of a fused-capillary , leading to a reversal of the electroosmotic flow ( EOF ) .
	manualset3
263396	3	426693	16	NULL	NULL	NULL	NULL	positive charge	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the running process , CB ( 7 ) bears a positive charge in the pH range of 2.5-7 .5 and can be adsorbed onto the inner wall of a fused-capillary , leading to a reversal of the electroosmotic flow ( EOF ) .
	manualset3
263397	4	426693	16	NULL	NULL	NULL	NULL	pH range	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the running process , CB ( 7 ) bears a positive charge in the pH range of 2.5-7 .5 and can be adsorbed onto the inner wall of a fused-capillary , leading to a reversal of the electroosmotic flow ( EOF ) .
	manualset3
263398	5	426693	16	NULL	NULL	NULL	NULL	2.5-7 .5	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the running process , CB ( 7 ) bears a positive charge in the pH range of 2.5-7 .5 and can be adsorbed onto the inner wall of a fused-capillary , leading to a reversal of the electroosmotic flow ( EOF ) .
	manualset3
263399	6	426693	16	NULL	NULL	NULL	NULL	inner wall	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the running process , CB ( 7 ) bears a positive charge in the pH range of 2.5-7 .5 and can be adsorbed onto the inner wall of a fused-capillary , leading to a reversal of the electroosmotic flow ( EOF ) .
	manualset3
263400	7	426693	16	NULL	NULL	NULL	NULL	reversal	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the running process , CB ( 7 ) bears a positive charge in the pH range of 2.5-7 .5 and can be adsorbed onto the inner wall of a fused-capillary , leading to a reversal of the electroosmotic flow ( EOF ) .
	manualset3
263401	8	426693	16	NULL	NULL	NULL	NULL	electroosmotic flow ( EOF )	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the running process , CB ( 7 ) bears a positive charge in the pH range of 2.5-7 .5 and can be adsorbed onto the inner wall of a fused-capillary , leading to a reversal of the electroosmotic flow ( EOF ) .
	manualset3
263402	1	426694	16	NULL	NULL	NULL	NULL	time period	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the same time period , mean melatonin levels increased in young women ( from 16.2 to 54.1 pg/mL , p & lt ; .001 ) and older women ( from 10.0 to 23.5 pg/mL , p & lt ; .001 ) , being lowest among the older poor sleepers ( from 20 : 00 to 24 : 00 h , p & lt ; .05 vs. young women ) .
	manualset3
263403	2	426694	16	NULL	NULL	NULL	NULL	mean melatonin levels	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the same time period , mean melatonin levels increased in young women ( from 16.2 to 54.1 pg/mL , p & lt ; .001 ) and older women ( from 10.0 to 23.5 pg/mL , p & lt ; .001 ) , being lowest among the older poor sleepers ( from 20 : 00 to 24 : 00 h , p & lt ; .05 vs. young women ) .
	manualset3
263404	3	426694	16	NULL	NULL	NULL	NULL	young women	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the same time period , mean melatonin levels increased in young women ( from 16.2 to 54.1 pg/mL , p & lt ; .001 ) and older women ( from 10.0 to 23.5 pg/mL , p & lt ; .001 ) , being lowest among the older poor sleepers ( from 20 : 00 to 24 : 00 h , p & lt ; .05 vs. young women ) .
	manualset3
263405	4	426694	16	NULL	NULL	NULL	NULL	16.2 to 54.1 pg/mL	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the same time period , mean melatonin levels increased in young women ( from 16.2 to 54.1 pg/mL , p & lt ; .001 ) and older women ( from 10.0 to 23.5 pg/mL , p & lt ; .001 ) , being lowest among the older poor sleepers ( from 20 : 00 to 24 : 00 h , p & lt ; .05 vs. young women ) .
	manualset3
263406	5	426694	16	NULL	NULL	NULL	NULL	p & lt ; .001	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the same time period , mean melatonin levels increased in young women ( from 16.2 to 54.1 pg/mL , p & lt ; .001 ) and older women ( from 10.0 to 23.5 pg/mL , p & lt ; .001 ) , being lowest among the older poor sleepers ( from 20 : 00 to 24 : 00 h , p & lt ; .05 vs. young women ) .
	manualset3
263407	6	426694	16	NULL	NULL	NULL	NULL	older women	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the same time period , mean melatonin levels increased in young women ( from 16.2 to 54.1 pg/mL , p & lt ; .001 ) and older women ( from 10.0 to 23.5 pg/mL , p & lt ; .001 ) , being lowest among the older poor sleepers ( from 20 : 00 to 24 : 00 h , p & lt ; .05 vs. young women ) .
	manualset3
263408	7	426694	16	NULL	NULL	NULL	NULL	10.0 to 23.5 pg/mL	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the same time period , mean melatonin levels increased in young women ( from 16.2 to 54.1 pg/mL , p & lt ; .001 ) and older women ( from 10.0 to 23.5 pg/mL , p & lt ; .001 ) , being lowest among the older poor sleepers ( from 20 : 00 to 24 : 00 h , p & lt ; .05 vs. young women ) .
	manualset3
263409	8	426694	16	NULL	NULL	NULL	NULL	p & lt ; .001	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the same time period , mean melatonin levels increased in young women ( from 16.2 to 54.1 pg/mL , p & lt ; .001 ) and older women ( from 10.0 to 23.5 pg/mL , p & lt ; .001 ) , being lowest among the older poor sleepers ( from 20 : 00 to 24 : 00 h , p & lt ; .05 vs. young women ) .
	manualset3
263410	9	426694	16	NULL	NULL	NULL	NULL	older poor sleepers	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the same time period , mean melatonin levels increased in young women ( from 16.2 to 54.1 pg/mL , p & lt ; .001 ) and older women ( from 10.0 to 23.5 pg/mL , p & lt ; .001 ) , being lowest among the older poor sleepers ( from 20 : 00 to 24 : 00 h , p & lt ; .05 vs. young women ) .
	manualset3
263411	10	426694	16	NULL	NULL	NULL	NULL	20 : 00 to 24 : 00 h	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the same time period , mean melatonin levels increased in young women ( from 16.2 to 54.1 pg/mL , p & lt ; .001 ) and older women ( from 10.0 to 23.5 pg/mL , p & lt ; .001 ) , being lowest among the older poor sleepers ( from 20 : 00 to 24 : 00 h , p & lt ; .05 vs. young women ) .
	manualset3
263412	11	426694	16	NULL	NULL	NULL	NULL	p & lt ; .05	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the same time period , mean melatonin levels increased in young women ( from 16.2 to 54.1 pg/mL , p & lt ; .001 ) and older women ( from 10.0 to 23.5 pg/mL , p & lt ; .001 ) , being lowest among the older poor sleepers ( from 20 : 00 to 24 : 00 h , p & lt ; .05 vs. young women ) .
	manualset3
263413	12	426694	16	NULL	NULL	NULL	NULL	young women	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the same time period , mean melatonin levels increased in young women ( from 16.2 to 54.1 pg/mL , p & lt ; .001 ) and older women ( from 10.0 to 23.5 pg/mL , p & lt ; .001 ) , being lowest among the older poor sleepers ( from 20 : 00 to 24 : 00 h , p & lt ; .05 vs. young women ) .
	manualset3
265380	1	426695	16	NULL	NULL	NULL	NULL	stationary phase	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the stationary phase of this run , sucrose was preferentially converted to product , and the substrate was completely depleted after 35 h of the process .
	manualset3
265381	2	426695	16	NULL	NULL	NULL	NULL	run	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the stationary phase of this run , sucrose was preferentially converted to product , and the substrate was completely depleted after 35 h of the process .
	manualset3
265382	3	426695	16	NULL	NULL	NULL	NULL	sucrose	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the stationary phase of this run , sucrose was preferentially converted to product , and the substrate was completely depleted after 35 h of the process .
	manualset3
265383	4	426695	16	NULL	NULL	NULL	NULL	product	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the stationary phase of this run , sucrose was preferentially converted to product , and the substrate was completely depleted after 35 h of the process .
	manualset3
265384	5	426695	16	NULL	NULL	NULL	NULL	substrate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the stationary phase of this run , sucrose was preferentially converted to product , and the substrate was completely depleted after 35 h of the process .
	manualset3
265385	6	426695	16	NULL	NULL	NULL	NULL	35 h	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the stationary phase of this run , sucrose was preferentially converted to product , and the substrate was completely depleted after 35 h of the process .
	manualset3
265386	7	426695	16	NULL	NULL	NULL	NULL	process	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the stationary phase of this run , sucrose was preferentially converted to product , and the substrate was completely depleted after 35 h of the process .
	manualset3
265387	1	426696	16	NULL	NULL	NULL	NULL	treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the treatment the prolactin values decreased in all patients to an average of 1.7 % of the baseline levels .
	manualset3
265388	2	426696	16	NULL	NULL	NULL	NULL	prolactin values	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the treatment the prolactin values decreased in all patients to an average of 1.7 % of the baseline levels .
	manualset3
265389	3	426696	16	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the treatment the prolactin values decreased in all patients to an average of 1.7 % of the baseline levels .
	manualset3
265390	4	426696	16	NULL	NULL	NULL	NULL	average	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the treatment the prolactin values decreased in all patients to an average of 1.7 % of the baseline levels .
	manualset3
265391	5	426696	16	NULL	NULL	NULL	NULL	1.7 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the treatment the prolactin values decreased in all patients to an average of 1.7 % of the baseline levels .
	manualset3
265392	6	426696	16	NULL	NULL	NULL	NULL	baseline levels	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the treatment the prolactin values decreased in all patients to an average of 1.7 % of the baseline levels .
	manualset3
265393	1	426697	16	NULL	NULL	NULL	NULL	Oral glucose tolerance test	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Oral glucose tolerance test using 100 g of glucose and 100 g of oligosaccarides ) .
	manualset3
265394	2	426697	16	NULL	NULL	NULL	NULL	100 g	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Oral glucose tolerance test using 100 g of glucose and 100 g of oligosaccarides ) .
	manualset3
265395	3	426697	16	NULL	NULL	NULL	NULL	glucose	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Oral glucose tolerance test using 100 g of glucose and 100 g of oligosaccarides ) .
	manualset3
265396	4	426697	16	NULL	NULL	NULL	NULL	100 g	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Oral glucose tolerance test using 100 g of glucose and 100 g of oligosaccarides ) .
	manualset3
265397	5	426697	16	NULL	NULL	NULL	NULL	oligosaccarides	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Oral glucose tolerance test using 100 g of glucose and 100 g of oligosaccarides ) .
	manualset3
265398	1	426698	16	NULL	NULL	NULL	NULL	war	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the war in Croatia so far , more than 250 casualties having missile wounds of the brain , spinal chord and peripheral nervous system were admitted to the Neurosurgical Clinic , University Hospital-Rebro .
	manualset3
265399	2	426698	16	NULL	NULL	NULL	NULL	Croatia	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the war in Croatia so far , more than 250 casualties having missile wounds of the brain , spinal chord and peripheral nervous system were admitted to the Neurosurgical Clinic , University Hospital-Rebro .
	manualset3
265400	3	426698	16	NULL	NULL	NULL	NULL	250 casualties	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the war in Croatia so far , more than 250 casualties having missile wounds of the brain , spinal chord and peripheral nervous system were admitted to the Neurosurgical Clinic , University Hospital-Rebro .
	manualset3
265401	4	426698	16	NULL	NULL	NULL	NULL	missile wounds	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the war in Croatia so far , more than 250 casualties having missile wounds of the brain , spinal chord and peripheral nervous system were admitted to the Neurosurgical Clinic , University Hospital-Rebro .
	manualset3
265402	5	426698	16	NULL	NULL	NULL	NULL	brain	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the war in Croatia so far , more than 250 casualties having missile wounds of the brain , spinal chord and peripheral nervous system were admitted to the Neurosurgical Clinic , University Hospital-Rebro .
	manualset3
265403	6	426698	16	NULL	NULL	NULL	NULL	spinal chord	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the war in Croatia so far , more than 250 casualties having missile wounds of the brain , spinal chord and peripheral nervous system were admitted to the Neurosurgical Clinic , University Hospital-Rebro .
	manualset3
265797	7	426698	16	NULL	NULL	NULL	NULL	peripheral nervous system	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the war in Croatia so far , more than 250 casualties having missile wounds of the brain , spinal chord and peripheral nervous system were admitted to the Neurosurgical Clinic , University Hospital-Rebro .
	manualset3
265798	8	426698	16	NULL	NULL	NULL	NULL	Neurosurgical Clinic	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the war in Croatia so far , more than 250 casualties having missile wounds of the brain , spinal chord and peripheral nervous system were admitted to the Neurosurgical Clinic , University Hospital-Rebro .
	manualset3
265799	9	426698	16	NULL	NULL	NULL	NULL	University Hospital-Rebro	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During the war in Croatia so far , more than 250 casualties having missile wounds of the brain , spinal chord and peripheral nervous system were admitted to the Neurosurgical Clinic , University Hospital-Rebro .
	manualset3
265800	1	426699	16	NULL	NULL	NULL	NULL	period	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During this period , 28 B. cepacia isolates were obtained from clinical specimens , and 2 were obtained from environmental specimens ( i.e. , from a nebulizer solution and a nebulizer tube ) .
	manualset3
265801	2	426699	16	NULL	NULL	NULL	NULL	28	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During this period , 28 B. cepacia isolates were obtained from clinical specimens , and 2 were obtained from environmental specimens ( i.e. , from a nebulizer solution and a nebulizer tube ) .
	manualset3
265802	3	426699	16	NULL	NULL	NULL	NULL	B. cepacia isolates	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During this period , 28 B. cepacia isolates were obtained from clinical specimens , and 2 were obtained from environmental specimens ( i.e. , from a nebulizer solution and a nebulizer tube ) .
	manualset3
265803	4	426699	16	NULL	NULL	NULL	NULL	clinical specimens	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During this period , 28 B. cepacia isolates were obtained from clinical specimens , and 2 were obtained from environmental specimens ( i.e. , from a nebulizer solution and a nebulizer tube ) .
	manualset3
265804	5	426699	16	NULL	NULL	NULL	NULL	2	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During this period , 28 B. cepacia isolates were obtained from clinical specimens , and 2 were obtained from environmental specimens ( i.e. , from a nebulizer solution and a nebulizer tube ) .
	manualset3
265805	6	426699	16	NULL	NULL	NULL	NULL	environmental specimens	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During this period , 28 B. cepacia isolates were obtained from clinical specimens , and 2 were obtained from environmental specimens ( i.e. , from a nebulizer solution and a nebulizer tube ) .
	manualset3
265806	7	426699	16	NULL	NULL	NULL	NULL	nebulizer solution	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During this period , 28 B. cepacia isolates were obtained from clinical specimens , and 2 were obtained from environmental specimens ( i.e. , from a nebulizer solution and a nebulizer tube ) .
	manualset3
265807	8	426699	16	NULL	NULL	NULL	NULL	nebulizer tube	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During this period , 28 B. cepacia isolates were obtained from clinical specimens , and 2 were obtained from environmental specimens ( i.e. , from a nebulizer solution and a nebulizer tube ) .
	manualset3
265808	1	426700	16	NULL	NULL	NULL	NULL	period	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During this period changes in management have included an increase in the caesarean section rate and the continuing development of methods of intensive care for the newborn infants .
	manualset3
265809	2	426700	16	NULL	NULL	NULL	NULL	changes	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During this period changes in management have included an increase in the caesarean section rate and the continuing development of methods of intensive care for the newborn infants .
	manualset3
265810	3	426700	16	NULL	NULL	NULL	NULL	management	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During this period changes in management have included an increase in the caesarean section rate and the continuing development of methods of intensive care for the newborn infants .
	manualset3
265811	4	426700	16	NULL	NULL	NULL	NULL	 increase	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During this period changes in management have included an increase in the caesarean section rate and the continuing development of methods of intensive care for the newborn infants .
	manualset3
265812	5	426700	16	NULL	NULL	NULL	NULL	caesarean section rate	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During this period changes in management have included an increase in the caesarean section rate and the continuing development of methods of intensive care for the newborn infants .
	manualset3
265813	6	426700	16	NULL	NULL	NULL	NULL	continuing development	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During this period changes in management have included an increase in the caesarean section rate and the continuing development of methods of intensive care for the newborn infants .
	manualset3
265814	7	426700	16	NULL	NULL	NULL	NULL	methods	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During this period changes in management have included an increase in the caesarean section rate and the continuing development of methods of intensive care for the newborn infants .
	manualset3
265815	8	426700	16	NULL	NULL	NULL	NULL	intensive care	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During this period changes in management have included an increase in the caesarean section rate and the continuing development of methods of intensive care for the newborn infants .
	manualset3
265816	9	426700	16	NULL	NULL	NULL	NULL	newborn infants	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During this period changes in management have included an increase in the caesarean section rate and the continuing development of methods of intensive care for the newborn infants .
	manualset3
265817	1	426701	16	NULL	NULL	NULL	NULL	period	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During this period the average value of the nitrogen elimination rate was 3.30 g N m ( -2 ) d ( -1 ) .
	manualset3
265818	2	426701	16	NULL	NULL	NULL	NULL	average value	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During this period the average value of the nitrogen elimination rate was 3.30 g N m ( -2 ) d ( -1 ) .
	manualset3
265819	3	426701	16	NULL	NULL	NULL	NULL	nitrogen elimination rate	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During this period the average value of the nitrogen elimination rate was 3.30 g N m ( -2 ) d ( -1 ) .
	manualset3
265820	4	426701	16	NULL	NULL	NULL	NULL	3.30 g N m ( -2 ) d ( -1 )	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During this period the average value of the nitrogen elimination rate was 3.30 g N m ( -2 ) d ( -1 ) .
	manualset3
265821	1	426702	16	NULL	NULL	NULL	NULL	thoracotomy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During thoracotomy in April 2001 , a mass was seen to have invaded the diaphragm with remarkable pleural adhesion .
	manualset3
265822	2	426702	16	NULL	NULL	NULL	NULL	April 2001	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During thoracotomy in April 2001 , a mass was seen to have invaded the diaphragm with remarkable pleural adhesion .
	manualset3
265823	3	426702	16	NULL	NULL	NULL	NULL	mass	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During thoracotomy in April 2001 , a mass was seen to have invaded the diaphragm with remarkable pleural adhesion .
	manualset3
265824	4	426702	16	NULL	NULL	NULL	NULL	diaphragm	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During thoracotomy in April 2001 , a mass was seen to have invaded the diaphragm with remarkable pleural adhesion .
	manualset3
265825	5	426702	16	NULL	NULL	NULL	NULL	pleural adhesion	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During thoracotomy in April 2001 , a mass was seen to have invaded the diaphragm with remarkable pleural adhesion .
	manualset3
265826	1	426703	16	NULL	NULL	NULL	NULL	tooth development	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During tooth development , dental epithelial cells interact with extracellular matrix components , such as the basement membrane and enamel matrix .
	manualset3
265827	2	426703	16	NULL	NULL	NULL	NULL	dental epithelial cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During tooth development , dental epithelial cells interact with extracellular matrix components , such as the basement membrane and enamel matrix .
	manualset3
265828	3	426703	16	NULL	NULL	NULL	NULL	extracellular matrix components	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During tooth development , dental epithelial cells interact with extracellular matrix components , such as the basement membrane and enamel matrix .
	manualset3
265829	4	426703	16	NULL	NULL	NULL	NULL	basement membrane	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During tooth development , dental epithelial cells interact with extracellular matrix components , such as the basement membrane and enamel matrix .
	manualset3
265830	5	426703	16	NULL	NULL	NULL	NULL	enamel matrix	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During tooth development , dental epithelial cells interact with extracellular matrix components , such as the basement membrane and enamel matrix .
	manualset3
265831	1	426704	16	NULL	NULL	NULL	NULL	tumor growth	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During tumor growth , anorexia and reduced food intake are among the major causes leading to malnutrition and eventually cachexia , which negatively affect patients ' outcome .
	manualset3
266669	2	426704	16	NULL	NULL	NULL	NULL	anorexia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During tumor growth , anorexia and reduced food intake are among the major causes leading to malnutrition and eventually cachexia , which negatively affect patients ' outcome .
	manualset3
266670	3	426704	16	NULL	NULL	NULL	NULL	reduced food intake	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During tumor growth , anorexia and reduced food intake are among the major causes leading to malnutrition and eventually cachexia , which negatively affect patients ' outcome .
	manualset3
266671	4	426704	16	NULL	NULL	NULL	NULL	major causes	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During tumor growth , anorexia and reduced food intake are among the major causes leading to malnutrition and eventually cachexia , which negatively affect patients ' outcome .
	manualset3
266672	5	426704	16	NULL	NULL	NULL	NULL	malnutrition	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During tumor growth , anorexia and reduced food intake are among the major causes leading to malnutrition and eventually cachexia , which negatively affect patients ' outcome .
	manualset3
266673	6	426704	16	NULL	NULL	NULL	NULL	cachexia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During tumor growth , anorexia and reduced food intake are among the major causes leading to malnutrition and eventually cachexia , which negatively affect patients ' outcome .
	manualset3
266674	7	426704	16	NULL	NULL	NULL	NULL	patients ' outcome	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During tumor growth , anorexia and reduced food intake are among the major causes leading to malnutrition and eventually cachexia , which negatively affect patients ' outcome .
	manualset3
266668	1	426705	16	NULL	NULL	NULL	NULL	unsaturated flow	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During unsaturated flow , P and Fe declined dramatically in the High-P zones ( P & lt ; 1 mg/l , Fe & lt ; 0.2 mg/l ) , whereas concentrations remained about the same during saturated and unsaturated flow in the Below zones .
	manualset3
266675	2	426705	16	NULL	NULL	NULL	NULL	P	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During unsaturated flow , P and Fe declined dramatically in the High-P zones ( P & lt ; 1 mg/l , Fe & lt ; 0.2 mg/l ) , whereas concentrations remained about the same during saturated and unsaturated flow in the Below zones .
	manualset3
266676	3	426705	16	NULL	NULL	NULL	NULL	Fe	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During unsaturated flow , P and Fe declined dramatically in the High-P zones ( P & lt ; 1 mg/l , Fe & lt ; 0.2 mg/l ) , whereas concentrations remained about the same during saturated and unsaturated flow in the Below zones .
	manualset3
266677	4	426705	16	NULL	NULL	NULL	NULL	High-P zones	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During unsaturated flow , P and Fe declined dramatically in the High-P zones ( P & lt ; 1 mg/l , Fe & lt ; 0.2 mg/l ) , whereas concentrations remained about the same during saturated and unsaturated flow in the Below zones .
	manualset3
266678	5	426705	16	NULL	NULL	NULL	NULL	P & lt ; 1 mg/l	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During unsaturated flow , P and Fe declined dramatically in the High-P zones ( P & lt ; 1 mg/l , Fe & lt ; 0.2 mg/l ) , whereas concentrations remained about the same during saturated and unsaturated flow in the Below zones .
	manualset3
266679	6	426705	16	NULL	NULL	NULL	NULL	Fe & lt ; 0.2 mg/l	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During unsaturated flow , P and Fe declined dramatically in the High-P zones ( P & lt ; 1 mg/l , Fe & lt ; 0.2 mg/l ) , whereas concentrations remained about the same during saturated and unsaturated flow in the Below zones .
	manualset3
266680	7	426705	16	NULL	NULL	NULL	NULL	concentrations	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During unsaturated flow , P and Fe declined dramatically in the High-P zones ( P & lt ; 1 mg/l , Fe & lt ; 0.2 mg/l ) , whereas concentrations remained about the same during saturated and unsaturated flow in the Below zones .
	manualset3
266681	8	426705	16	NULL	NULL	NULL	NULL	saturated flow	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During unsaturated flow , P and Fe declined dramatically in the High-P zones ( P & lt ; 1 mg/l , Fe & lt ; 0.2 mg/l ) , whereas concentrations remained about the same during saturated and unsaturated flow in the Below zones .
	manualset3
266682	9	426705	16	NULL	NULL	NULL	NULL	unsaturated flow	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During unsaturated flow , P and Fe declined dramatically in the High-P zones ( P & lt ; 1 mg/l , Fe & lt ; 0.2 mg/l ) , whereas concentrations remained about the same during saturated and unsaturated flow in the Below zones .
	manualset3
266683	10	426705	16	NULL	NULL	NULL	NULL	Below zones	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During unsaturated flow , P and Fe declined dramatically in the High-P zones ( P & lt ; 1 mg/l , Fe & lt ; 0.2 mg/l ) , whereas concentrations remained about the same during saturated and unsaturated flow in the Below zones .
	manualset3
266684	1	426706	16	NULL	NULL	NULL	NULL	uptake	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During uptake , ARH directly binds to the FxNPxY signal in the cytoplasmic tail of LDLR .
	manualset3
266685	2	426706	16	NULL	NULL	NULL	NULL	ARH	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During uptake , ARH directly binds to the FxNPxY signal in the cytoplasmic tail of LDLR .
	manualset3
266686	3	426706	16	NULL	NULL	NULL	NULL	FxNPxY signal	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During uptake , ARH directly binds to the FxNPxY signal in the cytoplasmic tail of LDLR .
	manualset3
266687	4	426706	16	NULL	NULL	NULL	NULL	cytoplasmic tail	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During uptake , ARH directly binds to the FxNPxY signal in the cytoplasmic tail of LDLR .
	manualset3
266688	5	426706	16	NULL	NULL	NULL	NULL	LDLR	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During uptake , ARH directly binds to the FxNPxY signal in the cytoplasmic tail of LDLR .
	manualset3
266689	1	426707	16	NULL	NULL	NULL	NULL	uptake of bacteria	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During uptake of bacteria or yeast , PHcrac-GFP , a probe that binds to membranes enriched in PI ( 3 , 4 , 5 ) P ( 3 ) and PI ( 3 , 4 ) P ( 2 ) , always labeled the nascent phagosome and faded shortly after it sealed .
	manualset3
266690	2	426707	16	NULL	NULL	NULL	NULL	uptake of yeast	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During uptake of bacteria or yeast , PHcrac-GFP , a probe that binds to membranes enriched in PI ( 3 , 4 , 5 ) P ( 3 ) and PI ( 3 , 4 ) P ( 2 ) , always labeled the nascent phagosome and faded shortly after it sealed .
	manualset3
266691	3	426707	16	NULL	NULL	NULL	NULL	PHcrac-GFP	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During uptake of bacteria or yeast , PHcrac-GFP , a probe that binds to membranes enriched in PI ( 3 , 4 , 5 ) P ( 3 ) and PI ( 3 , 4 ) P ( 2 ) , always labeled the nascent phagosome and faded shortly after it sealed .
	manualset3
266692	4	426707	16	NULL	NULL	NULL	NULL	probe	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During uptake of bacteria or yeast , PHcrac-GFP , a probe that binds to membranes enriched in PI ( 3 , 4 , 5 ) P ( 3 ) and PI ( 3 , 4 ) P ( 2 ) , always labeled the nascent phagosome and faded shortly after it sealed .
	manualset3
266693	5	426707	16	NULL	NULL	NULL	NULL	membranes	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During uptake of bacteria or yeast , PHcrac-GFP , a probe that binds to membranes enriched in PI ( 3 , 4 , 5 ) P ( 3 ) and PI ( 3 , 4 ) P ( 2 ) , always labeled the nascent phagosome and faded shortly after it sealed .
	manualset3
266694	6	426707	16	NULL	NULL	NULL	NULL	PI ( 3 , 4 , 5 ) P ( 3 )	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During uptake of bacteria or yeast , PHcrac-GFP , a probe that binds to membranes enriched in PI ( 3 , 4 , 5 ) P ( 3 ) and PI ( 3 , 4 ) P ( 2 ) , always labeled the nascent phagosome and faded shortly after it sealed .
	manualset3
266695	7	426707	16	NULL	NULL	NULL	NULL	 PI ( 3 , 4 ) P ( 2 )	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During uptake of bacteria or yeast , PHcrac-GFP , a probe that binds to membranes enriched in PI ( 3 , 4 , 5 ) P ( 3 ) and PI ( 3 , 4 ) P ( 2 ) , always labeled the nascent phagosome and faded shortly after it sealed .
	manualset3
266696	8	426707	16	NULL	NULL	NULL	NULL	nascent phagosome	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During uptake of bacteria or yeast , PHcrac-GFP , a probe that binds to membranes enriched in PI ( 3 , 4 , 5 ) P ( 3 ) and PI ( 3 , 4 ) P ( 2 ) , always labeled the nascent phagosome and faded shortly after it sealed .
	manualset3
266697	1	426708	16	NULL	NULL	NULL	NULL	Orbitol sinus venography	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Orbital and cavernous sinus venography via frontal vein ) .
	manualset3
266698	2	426708	16	NULL	NULL	NULL	NULL	cavernous sinus venography	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Orbital and cavernous sinus venography via frontal vein ) .
	manualset3
266699	3	426708	16	NULL	NULL	NULL	NULL	frontal vein	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Orbital and cavernous sinus venography via frontal vein ) .
	manualset3
266700	1	426709	16	NULL	NULL	NULL	NULL	winter	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During winter , DHEA-S levels were maintained low and constant over lifetime .
	manualset3
266701	2	426709	16	NULL	NULL	NULL	NULL	DHEA-S levels	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During winter , DHEA-S levels were maintained low and constant over lifetime .
	manualset3
266702	3	426709	16	NULL	NULL	NULL	NULL	over lifetime	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	During winter , DHEA-S levels were maintained low and constant over lifetime .
	manualset3
266703	1	426710	16	NULL	NULL	NULL	NULL	DxS kits	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DxS kits detect mutations in oncogenes associated with cancer drug response .
	manualset3
266704	2	426710	16	NULL	NULL	NULL	NULL	mutations	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DxS kits detect mutations in oncogenes associated with cancer drug response .
	manualset3
266705	3	426710	16	NULL	NULL	NULL	NULL	oncogenes	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DxS kits detect mutations in oncogenes associated with cancer drug response .
	manualset3
266706	4	426710	16	NULL	NULL	NULL	NULL	cancer drug response	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	DxS kits detect mutations in oncogenes associated with cancer drug response .
	manualset3
266707	1	426711	16	NULL	NULL	NULL	NULL	Dynal M-270 magnetic beads	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynal M-270 magnetic beads were chosen to further study the system as a model for capturing and identifying the targets of ampicillin , PBPs that were specifically and covalently bound to the immobilized ampicillin .
	manualset3
266708	2	426711	16	NULL	NULL	NULL	NULL	study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynal M-270 magnetic beads were chosen to further study the system as a model for capturing and identifying the targets of ampicillin , PBPs that were specifically and covalently bound to the immobilized ampicillin .
	manualset3
266709	3	426711	16	NULL	NULL	NULL	NULL	system	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynal M-270 magnetic beads were chosen to further study the system as a model for capturing and identifying the targets of ampicillin , PBPs that were specifically and covalently bound to the immobilized ampicillin .
	manualset3
266710	4	426711	16	NULL	NULL	NULL	NULL	model	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynal M-270 magnetic beads were chosen to further study the system as a model for capturing and identifying the targets of ampicillin , PBPs that were specifically and covalently bound to the immobilized ampicillin .
	manualset3
266711	5	426711	16	NULL	NULL	NULL	NULL	targets	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynal M-270 magnetic beads were chosen to further study the system as a model for capturing and identifying the targets of ampicillin , PBPs that were specifically and covalently bound to the immobilized ampicillin .
	manualset3
266712	6	426711	16	NULL	NULL	NULL	NULL	ampicillin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynal M-270 magnetic beads were chosen to further study the system as a model for capturing and identifying the targets of ampicillin , PBPs that were specifically and covalently bound to the immobilized ampicillin .
	manualset3
266713	7	426711	16	NULL	NULL	NULL	NULL	PBPs	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynal M-270 magnetic beads were chosen to further study the system as a model for capturing and identifying the targets of ampicillin , PBPs that were specifically and covalently bound to the immobilized ampicillin .
	manualset3
266714	8	426711	16	NULL	NULL	NULL	NULL	immobilized ampicillin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynal M-270 magnetic beads were chosen to further study the system as a model for capturing and identifying the targets of ampicillin , PBPs that were specifically and covalently bound to the immobilized ampicillin .
	manualset3
266715	1	426712	16	NULL	NULL	NULL	NULL	Dynalog files	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynalog files are recorded for each delivery and converted into DMLC field files using in-house program .
	manualset3
266716	2	426712	16	NULL	NULL	NULL	NULL	delivery	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynalog files are recorded for each delivery and converted into DMLC field files using in-house program .
	manualset3
266717	3	426712	16	NULL	NULL	NULL	NULL	DMLC field files	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynalog files are recorded for each delivery and converted into DMLC field files using in-house program .
	manualset3
266718	4	426712	16	NULL	NULL	NULL	NULL	in-house program	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynalog files are recorded for each delivery and converted into DMLC field files using in-house program .
	manualset3
266719	1	426713	16	NULL	NULL	NULL	NULL	Dynamic aspects	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamic aspects concerned with the mechanism of separating motile sperm from nonmotile sperm , leukocytes , and debris with the use of high-density Percoll gradients .
	manualset3
266720	2	426713	16	NULL	NULL	NULL	NULL	mechanism	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamic aspects concerned with the mechanism of separating motile sperm from nonmotile sperm , leukocytes , and debris with the use of high-density Percoll gradients .
	manualset3
266721	3	426713	16	NULL	NULL	NULL	NULL	motile sperm	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamic aspects concerned with the mechanism of separating motile sperm from nonmotile sperm , leukocytes , and debris with the use of high-density Percoll gradients .
	manualset3
266722	4	426713	16	NULL	NULL	NULL	NULL	nonmotile sperm	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamic aspects concerned with the mechanism of separating motile sperm from nonmotile sperm , leukocytes , and debris with the use of high-density Percoll gradients .
	manualset3
266723	5	426713	16	NULL	NULL	NULL	NULL	leukocytes	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamic aspects concerned with the mechanism of separating motile sperm from nonmotile sperm , leukocytes , and debris with the use of high-density Percoll gradients .
	manualset3
266724	6	426713	16	NULL	NULL	NULL	NULL	debris	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamic aspects concerned with the mechanism of separating motile sperm from nonmotile sperm , leukocytes , and debris with the use of high-density Percoll gradients .
	manualset3
266725	7	426713	16	NULL	NULL	NULL	NULL	 high-density Percoll gradients	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamic aspects concerned with the mechanism of separating motile sperm from nonmotile sperm , leukocytes , and debris with the use of high-density Percoll gradients .
	manualset3
266726	1	426714	16	NULL	NULL	NULL	NULL	Dynamic molecular modeling	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamic molecular modeling of the 11th structural repeat of human alpha II spectrin incorporating the various mutations suggests that the calpain cleavage site with its flanking calmodulin binding domain interrupts helix C of alpha II spectrin 's 11th repetitive unit without significantly disrupting the repeat 's triple-helical motif .
	manualset3
266727	2	426714	16	NULL	NULL	NULL	NULL	11th structural repeat	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamic molecular modeling of the 11th structural repeat of human alpha II spectrin incorporating the various mutations suggests that the calpain cleavage site with its flanking calmodulin binding domain interrupts helix C of alpha II spectrin 's 11th repetitive unit without significantly disrupting the repeat 's triple-helical motif .
	manualset3
266728	3	426714	16	NULL	NULL	NULL	NULL	human alpha II spectrin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamic molecular modeling of the 11th structural repeat of human alpha II spectrin incorporating the various mutations suggests that the calpain cleavage site with its flanking calmodulin binding domain interrupts helix C of alpha II spectrin 's 11th repetitive unit without significantly disrupting the repeat 's triple-helical motif .
	manualset3
266729	4	426714	16	NULL	NULL	NULL	NULL	various mutations	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamic molecular modeling of the 11th structural repeat of human alpha II spectrin incorporating the various mutations suggests that the calpain cleavage site with its flanking calmodulin binding domain interrupts helix C of alpha II spectrin 's 11th repetitive unit without significantly disrupting the repeat 's triple-helical motif .
	manualset3
266730	5	426714	16	NULL	NULL	NULL	NULL	calpain cleavage site	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamic molecular modeling of the 11th structural repeat of human alpha II spectrin incorporating the various mutations suggests that the calpain cleavage site with its flanking calmodulin binding domain interrupts helix C of alpha II spectrin 's 11th repetitive unit without significantly disrupting the repeat 's triple-helical motif .
	manualset3
266731	6	426714	16	NULL	NULL	NULL	NULL	calmodulin binding domain	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamic molecular modeling of the 11th structural repeat of human alpha II spectrin incorporating the various mutations suggests that the calpain cleavage site with its flanking calmodulin binding domain interrupts helix C of alpha II spectrin 's 11th repetitive unit without significantly disrupting the repeat 's triple-helical motif .
	manualset3
266732	7	426714	16	NULL	NULL	NULL	NULL	helix C	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamic molecular modeling of the 11th structural repeat of human alpha II spectrin incorporating the various mutations suggests that the calpain cleavage site with its flanking calmodulin binding domain interrupts helix C of alpha II spectrin 's 11th repetitive unit without significantly disrupting the repeat 's triple-helical motif .
	manualset3
266733	8	426714	16	NULL	NULL	NULL	NULL	alpha II spectrin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamic molecular modeling of the 11th structural repeat of human alpha II spectrin incorporating the various mutations suggests that the calpain cleavage site with its flanking calmodulin binding domain interrupts helix C of alpha II spectrin 's 11th repetitive unit without significantly disrupting the repeat 's triple-helical motif .
	manualset3
266734	9	426714	16	NULL	NULL	NULL	NULL	11th repetitive unit	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamic molecular modeling of the 11th structural repeat of human alpha II spectrin incorporating the various mutations suggests that the calpain cleavage site with its flanking calmodulin binding domain interrupts helix C of alpha II spectrin 's 11th repetitive unit without significantly disrupting the repeat 's triple-helical motif .
	manualset3
266735	10	426714	16	NULL	NULL	NULL	NULL	repeat	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamic molecular modeling of the 11th structural repeat of human alpha II spectrin incorporating the various mutations suggests that the calpain cleavage site with its flanking calmodulin binding domain interrupts helix C of alpha II spectrin 's 11th repetitive unit without significantly disrupting the repeat 's triple-helical motif .
	manualset3
266736	11	426714	16	NULL	NULL	NULL	NULL	triple-helical motif	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamic molecular modeling of the 11th structural repeat of human alpha II spectrin incorporating the various mutations suggests that the calpain cleavage site with its flanking calmodulin binding domain interrupts helix C of alpha II spectrin 's 11th repetitive unit without significantly disrupting the repeat 's triple-helical motif .
	manualset3
266737	1	426715	16	NULL	NULL	NULL	NULL	Dynamic stability	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamic stability after ACL injury : who can hop ?
	manualset3
266738	2	426715	16	NULL	NULL	NULL	NULL	ACL injury	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamic stability after ACL injury : who can hop ?
	manualset3
266739	1	426716	16	NULL	NULL	NULL	NULL	Dynamic surface tension	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamic surface tension is measured through the differential pressure across the air/liquid interface of repeatedly growing and detaching drops .
	manualset3
266740	2	426716	16	NULL	NULL	NULL	NULL	differential pressure	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamic surface tension is measured through the differential pressure across the air/liquid interface of repeatedly growing and detaching drops .
	manualset3
266741	3	426716	16	NULL	NULL	NULL	NULL	air/liquid interface	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamic surface tension is measured through the differential pressure across the air/liquid interface of repeatedly growing and detaching drops .
	manualset3
266742	4	426716	16	NULL	NULL	NULL	NULL	drops	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamic surface tension is measured through the differential pressure across the air/liquid interface of repeatedly growing and detaching drops .
	manualset3
266743	1	426717	16	NULL	NULL	NULL	NULL	Organ transplantation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Organ transplantation -- nursing aspects of care ) .
	manualset3
266744	2	426717	16	NULL	NULL	NULL	NULL	nursing aspects	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Organ transplantation -- nursing aspects of care ) .
	manualset3
266745	3	426717	16	NULL	NULL	NULL	NULL	care	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Organ transplantation -- nursing aspects of care ) .
	manualset3
266746	1	426718	16	NULL	NULL	NULL	NULL	Dynamic vagal control	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamic vagal control of pacemaker activity in the mammalian sinoatrial node .
	manualset3
266747	2	426718	16	NULL	NULL	NULL	NULL	pacemaker activity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamic vagal control of pacemaker activity in the mammalian sinoatrial node .
	manualset3
266748	3	426718	16	NULL	NULL	NULL	NULL	mammalian sinoatrial node	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamic vagal control of pacemaker activity in the mammalian sinoatrial node .
	manualset3
266749	1	426719	16	NULL	NULL	NULL	NULL	Dynamics	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamics of learning in multilayer perceptrons near singularities .
	manualset3
266750	2	426719	16	NULL	NULL	NULL	NULL	learning	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamics of learning in multilayer perceptrons near singularities .
	manualset3
266751	3	426719	16	NULL	NULL	NULL	NULL	multilayer perceptrons	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamics of learning in multilayer perceptrons near singularities .
	manualset3
266752	4	426719	16	NULL	NULL	NULL	NULL	singularities	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dynamics of learning in multilayer perceptrons near singularities .
	manualset3
266753	1	426720	16	NULL	NULL	NULL	NULL	Dysadherin expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysadherin expression in head and neck squamous cell carcinoma : association with lymphangiogenesis and prognostic significance .
	manualset3
266754	2	426720	16	NULL	NULL	NULL	NULL	head and neck squamous cell carcinoma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysadherin expression in head and neck squamous cell carcinoma : association with lymphangiogenesis and prognostic significance .
	manualset3
266755	3	426720	16	NULL	NULL	NULL	NULL	association	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysadherin expression in head and neck squamous cell carcinoma : association with lymphangiogenesis and prognostic significance .
	manualset3
266756	4	426720	16	NULL	NULL	NULL	NULL	lymphangiogenesis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysadherin expression in head and neck squamous cell carcinoma : association with lymphangiogenesis and prognostic significance .
	manualset3
266757	5	426720	16	NULL	NULL	NULL	NULL	prognostic significance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysadherin expression in head and neck squamous cell carcinoma : association with lymphangiogenesis and prognostic significance .
	manualset3
266758	1	426721	16	NULL	NULL	NULL	NULL	Dysentery	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysentery , plaque or parasitic disease ? ) .
	manualset3
266759	2	426721	16	NULL	NULL	NULL	NULL	plaque	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysentery , plaque or parasitic disease ? ) .
	manualset3
266760	3	426721	16	NULL	NULL	NULL	NULL	parasitic disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysentery , plaque or parasitic disease ? ) .
	manualset3
266761	1	426722	16	NULL	NULL	NULL	NULL	Dysfunction	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysfunction may concern one or more physiologic properties like tonus , motility , secretion , sometimes also resorption and digestion , or their interaction .
	manualset3
266762	2	426722	16	NULL	NULL	NULL	NULL	one	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysfunction may concern one or more physiologic properties like tonus , motility , secretion , sometimes also resorption and digestion , or their interaction .
	manualset3
266763	3	426722	16	NULL	NULL	NULL	NULL	physiologic properties	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysfunction may concern one or more physiologic properties like tonus , motility , secretion , sometimes also resorption and digestion , or their interaction .
	manualset3
266764	4	426722	16	NULL	NULL	NULL	NULL	tonus	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysfunction may concern one or more physiologic properties like tonus , motility , secretion , sometimes also resorption and digestion , or their interaction .
	manualset3
266765	5	426722	16	NULL	NULL	NULL	NULL	motility	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysfunction may concern one or more physiologic properties like tonus , motility , secretion , sometimes also resorption and digestion , or their interaction .
	manualset3
266766	6	426722	16	NULL	NULL	NULL	NULL	secretion	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysfunction may concern one or more physiologic properties like tonus , motility , secretion , sometimes also resorption and digestion , or their interaction .
	manualset3
266767	7	426722	16	NULL	NULL	NULL	NULL	resorption	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysfunction may concern one or more physiologic properties like tonus , motility , secretion , sometimes also resorption and digestion , or their interaction .
	manualset3
266768	8	426722	16	NULL	NULL	NULL	NULL	digestion	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysfunction may concern one or more physiologic properties like tonus , motility , secretion , sometimes also resorption and digestion , or their interaction .
	manualset3
266769	9	426722	16	NULL	NULL	NULL	NULL	interaction	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysfunction may concern one or more physiologic properties like tonus , motility , secretion , sometimes also resorption and digestion , or their interaction .
	manualset3
266770	1	426723	16	NULL	NULL	NULL	NULL	Dysmorphic neurons	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysmorphic neurons in both FCD Type II variants showed significantly increased diameter of their cell bodies and nuclei .
	manualset3
266771	2	426723	16	NULL	NULL	NULL	NULL	FCD Type II variants	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysmorphic neurons in both FCD Type II variants showed significantly increased diameter of their cell bodies and nuclei .
	manualset3
266772	3	426723	16	NULL	NULL	NULL	NULL	increased diameter	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysmorphic neurons in both FCD Type II variants showed significantly increased diameter of their cell bodies and nuclei .
	manualset3
266773	4	426723	16	NULL	NULL	NULL	NULL	cell bodies	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysmorphic neurons in both FCD Type II variants showed significantly increased diameter of their cell bodies and nuclei .
	manualset3
266774	5	426723	16	NULL	NULL	NULL	NULL	nuclei	CellComponent												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysmorphic neurons in both FCD Type II variants showed significantly increased diameter of their cell bodies and nuclei .
	manualset3
266775	1	426724	16	NULL	NULL	NULL	NULL	Dysmyelination	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysmyelination in mice and the proteolipid protein gene family .
	manualset3
266776	2	426724	16	NULL	NULL	NULL	NULL	mice	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysmyelination in mice and the proteolipid protein gene family .
	manualset3
266777	3	426724	16	NULL	NULL	NULL	NULL	proteolipid protein gene family	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysmyelination in mice and the proteolipid protein gene family .
	manualset3
266778	1	426725	16	NULL	NULL	NULL	NULL	Organization	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Organization of blood transfusion service in smaller hospitals ) .
	manualset3
266779	2	426725	16	NULL	NULL	NULL	NULL	blood transfusion service	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Organization of blood transfusion service in smaller hospitals ) .
	manualset3
266780	3	426725	16	NULL	NULL	NULL	NULL	smaller hospitals	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Organization of blood transfusion service in smaller hospitals ) .
	manualset3
266781	1	426726	16	NULL	NULL	NULL	NULL	Dysphoria	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysphoria and immune status in postpartum women .
	manualset3
266782	2	426726	16	NULL	NULL	NULL	NULL	immune status	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysphoria and immune status in postpartum women .
	manualset3
266783	3	426726	16	NULL	NULL	NULL	NULL	postpartum women	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysphoria and immune status in postpartum women .
	manualset3
266784	1	426727	16	NULL	NULL	NULL	NULL	Dysplasia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysplasia was confirmed on biopsy of 11 cases cytologically diagnosed as HGSIL ( 7 CINII/III and 4 CIN I ) , 19 cases cytologically diagnosed as LGSIL ( 6 CIN II/III and 13 CIN I ) , 35 cases of ASCUS ( 4 CIN II/III and 31 CIN I ) , and 2 cases of AGUS ( 1 CIN III and 1 CIN I ) .
	manualset3
266785	2	426727	16	NULL	NULL	NULL	NULL	biopsy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysplasia was confirmed on biopsy of 11 cases cytologically diagnosed as HGSIL ( 7 CINII/III and 4 CIN I ) , 19 cases cytologically diagnosed as LGSIL ( 6 CIN II/III and 13 CIN I ) , 35 cases of ASCUS ( 4 CIN II/III and 31 CIN I ) , and 2 cases of AGUS ( 1 CIN III and 1 CIN I ) .
	manualset3
266786	3	426727	16	NULL	NULL	NULL	NULL	11 cases	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysplasia was confirmed on biopsy of 11 cases cytologically diagnosed as HGSIL ( 7 CINII/III and 4 CIN I ) , 19 cases cytologically diagnosed as LGSIL ( 6 CIN II/III and 13 CIN I ) , 35 cases of ASCUS ( 4 CIN II/III and 31 CIN I ) , and 2 cases of AGUS ( 1 CIN III and 1 CIN I ) .
	manualset3
266787	4	426727	16	NULL	NULL	NULL	NULL	HGSIL ( 7 CINII/III and 4 CIN I )	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysplasia was confirmed on biopsy of 11 cases cytologically diagnosed as HGSIL ( 7 CINII/III and 4 CIN I ) , 19 cases cytologically diagnosed as LGSIL ( 6 CIN II/III and 13 CIN I ) , 35 cases of ASCUS ( 4 CIN II/III and 31 CIN I ) , and 2 cases of AGUS ( 1 CIN III and 1 CIN I ) .
	manualset3
266788	5	426727	16	NULL	NULL	NULL	NULL	19 cases	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysplasia was confirmed on biopsy of 11 cases cytologically diagnosed as HGSIL ( 7 CINII/III and 4 CIN I ) , 19 cases cytologically diagnosed as LGSIL ( 6 CIN II/III and 13 CIN I ) , 35 cases of ASCUS ( 4 CIN II/III and 31 CIN I ) , and 2 cases of AGUS ( 1 CIN III and 1 CIN I ) .
	manualset3
266789	6	426727	16	NULL	NULL	NULL	NULL	LGSIL ( 6 CIN II/III and 13 CIN I )	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysplasia was confirmed on biopsy of 11 cases cytologically diagnosed as HGSIL ( 7 CINII/III and 4 CIN I ) , 19 cases cytologically diagnosed as LGSIL ( 6 CIN II/III and 13 CIN I ) , 35 cases of ASCUS ( 4 CIN II/III and 31 CIN I ) , and 2 cases of AGUS ( 1 CIN III and 1 CIN I ) .
	manualset3
266790	7	426727	16	NULL	NULL	NULL	NULL	35 cases	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysplasia was confirmed on biopsy of 11 cases cytologically diagnosed as HGSIL ( 7 CINII/III and 4 CIN I ) , 19 cases cytologically diagnosed as LGSIL ( 6 CIN II/III and 13 CIN I ) , 35 cases of ASCUS ( 4 CIN II/III and 31 CIN I ) , and 2 cases of AGUS ( 1 CIN III and 1 CIN I ) .
	manualset3
266791	8	426727	16	NULL	NULL	NULL	NULL	ASCUS ( 4 CIN II/III and 31 CIN I )	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysplasia was confirmed on biopsy of 11 cases cytologically diagnosed as HGSIL ( 7 CINII/III and 4 CIN I ) , 19 cases cytologically diagnosed as LGSIL ( 6 CIN II/III and 13 CIN I ) , 35 cases of ASCUS ( 4 CIN II/III and 31 CIN I ) , and 2 cases of AGUS ( 1 CIN III and 1 CIN I ) .
	manualset3
266792	9	426727	16	NULL	NULL	NULL	NULL	2 cases	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysplasia was confirmed on biopsy of 11 cases cytologically diagnosed as HGSIL ( 7 CINII/III and 4 CIN I ) , 19 cases cytologically diagnosed as LGSIL ( 6 CIN II/III and 13 CIN I ) , 35 cases of ASCUS ( 4 CIN II/III and 31 CIN I ) , and 2 cases of AGUS ( 1 CIN III and 1 CIN I ) .
	manualset3
266793	10	426727	16	NULL	NULL	NULL	NULL	AGUS ( 1 CIN III and 1 CIN I )	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Dysplasia was confirmed on biopsy of 11 cases cytologically diagnosed as HGSIL ( 7 CINII/III and 4 CIN I ) , 19 cases cytologically diagnosed as LGSIL ( 6 CIN II/III and 13 CIN I ) , 35 cases of ASCUS ( 4 CIN II/III and 31 CIN I ) , and 2 cases of AGUS ( 1 CIN III and 1 CIN I ) .
	manualset3
266797	1	426729	16	NULL	NULL	NULL	NULL	E-5 - ( 2-Bromovinyl ) -2 ' - deoxyuridylate ( BrvdUMP )	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E-5 - ( 2-Bromovinyl ) -2 ' - deoxyuridylate ( BrvdUMP ) , the first metabolite in the processing of the antiviral agent E-5 - ( 2-bromovinyl ) -2 ' - deoxyuridine ( BrvdUrd ) , is an excellent alternate substrate for dTMP synthetase .
	manualset3
266798	2	426729	16	NULL	NULL	NULL	NULL	first metabolite	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E-5 - ( 2-Bromovinyl ) -2 ' - deoxyuridylate ( BrvdUMP ) , the first metabolite in the processing of the antiviral agent E-5 - ( 2-bromovinyl ) -2 ' - deoxyuridine ( BrvdUrd ) , is an excellent alternate substrate for dTMP synthetase .
	manualset3
266799	3	426729	16	NULL	NULL	NULL	NULL	antiviral agent	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E-5 - ( 2-Bromovinyl ) -2 ' - deoxyuridylate ( BrvdUMP ) , the first metabolite in the processing of the antiviral agent E-5 - ( 2-bromovinyl ) -2 ' - deoxyuridine ( BrvdUrd ) , is an excellent alternate substrate for dTMP synthetase .
	manualset3
266800	4	426729	16	NULL	NULL	NULL	NULL	E-5 - ( 2-bromovinyl ) -2 ' - deoxyuridine ( BrvdUrd )	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E-5 - ( 2-Bromovinyl ) -2 ' - deoxyuridylate ( BrvdUMP ) , the first metabolite in the processing of the antiviral agent E-5 - ( 2-bromovinyl ) -2 ' - deoxyuridine ( BrvdUrd ) , is an excellent alternate substrate for dTMP synthetase .
	manualset3
266801	5	426729	16	NULL	NULL	NULL	NULL	substrate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E-5 - ( 2-Bromovinyl ) -2 ' - deoxyuridylate ( BrvdUMP ) , the first metabolite in the processing of the antiviral agent E-5 - ( 2-bromovinyl ) -2 ' - deoxyuridine ( BrvdUrd ) , is an excellent alternate substrate for dTMP synthetase .
	manualset3
266802	6	426729	16	NULL	NULL	NULL	NULL	dTMP synthetase	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E-5 - ( 2-Bromovinyl ) -2 ' - deoxyuridylate ( BrvdUMP ) , the first metabolite in the processing of the antiviral agent E-5 - ( 2-bromovinyl ) -2 ' - deoxyuridine ( BrvdUrd ) , is an excellent alternate substrate for dTMP synthetase .
	manualset3
266803	1	426730	16	NULL	NULL	NULL	NULL	E-I	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E-I and E-II did not depend on metal ions although activity of the latter was slightly stimulated by Mn2 + and Ca2 + in the range of 0.5-2 mM .
	manualset3
266804	2	426730	16	NULL	NULL	NULL	NULL	E-II	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E-I and E-II did not depend on metal ions although activity of the latter was slightly stimulated by Mn2 + and Ca2 + in the range of 0.5-2 mM .
	manualset3
266805	3	426730	16	NULL	NULL	NULL	NULL	metal ions	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E-I and E-II did not depend on metal ions although activity of the latter was slightly stimulated by Mn2 + and Ca2 + in the range of 0.5-2 mM .
	manualset3
266806	4	426730	16	NULL	NULL	NULL	NULL	activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E-I and E-II did not depend on metal ions although activity of the latter was slightly stimulated by Mn2 + and Ca2 + in the range of 0.5-2 mM .
	manualset3
266807	5	426730	16	NULL	NULL	NULL	NULL	Mn2 +	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E-I and E-II did not depend on metal ions although activity of the latter was slightly stimulated by Mn2 + and Ca2 + in the range of 0.5-2 mM .
	manualset3
266808	6	426730	16	NULL	NULL	NULL	NULL	Ca2 +	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E-I and E-II did not depend on metal ions although activity of the latter was slightly stimulated by Mn2 + and Ca2 + in the range of 0.5-2 mM .
	manualset3
266809	7	426730	16	NULL	NULL	NULL	NULL	range	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E-I and E-II did not depend on metal ions although activity of the latter was slightly stimulated by Mn2 + and Ca2 + in the range of 0.5-2 mM .
	manualset3
266810	8	426730	16	NULL	NULL	NULL	NULL	0.5-2 mM	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E-I and E-II did not depend on metal ions although activity of the latter was slightly stimulated by Mn2 + and Ca2 + in the range of 0.5-2 mM .
	manualset3
266811	1	426731	16	NULL	NULL	NULL	NULL	E-Phytol	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E-Phytol , phytone , bis ( 2-ethylhexyl ) phthalate and friedelin were isolated as active anti-inflammatory components inhibiting carrageenin-induced paw edema .
	manualset3
266812	2	426731	16	NULL	NULL	NULL	NULL	phytone	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E-Phytol , phytone , bis ( 2-ethylhexyl ) phthalate and friedelin were isolated as active anti-inflammatory components inhibiting carrageenin-induced paw edema .
	manualset3
266813	3	426731	16	NULL	NULL	NULL	NULL	 bis ( 2-ethylhexyl ) phthalate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E-Phytol , phytone , bis ( 2-ethylhexyl ) phthalate and friedelin were isolated as active anti-inflammatory components inhibiting carrageenin-induced paw edema .
	manualset3
266814	4	426731	16	NULL	NULL	NULL	NULL	friedelin	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E-Phytol , phytone , bis ( 2-ethylhexyl ) phthalate and friedelin were isolated as active anti-inflammatory components inhibiting carrageenin-induced paw edema .
	manualset3
266815	5	426731	16	NULL	NULL	NULL	NULL	anti-inflammatory components	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E-Phytol , phytone , bis ( 2-ethylhexyl ) phthalate and friedelin were isolated as active anti-inflammatory components inhibiting carrageenin-induced paw edema .
	manualset3
266816	6	426731	16	NULL	NULL	NULL	NULL	 carrageenin-induced paw edema	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E-Phytol , phytone , bis ( 2-ethylhexyl ) phthalate and friedelin were isolated as active anti-inflammatory components inhibiting carrageenin-induced paw edema .
	manualset3
266817	1	426732	16	NULL	NULL	NULL	NULL	E-cadherin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E-cadherin is a hallmark of epithelial-mesenchymal transition ( EMT ) , which plays a crucial role in cancer metastasis .
	manualset3
266818	2	426732	16	NULL	NULL	NULL	NULL	hallmark	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E-cadherin is a hallmark of epithelial-mesenchymal transition ( EMT ) , which plays a crucial role in cancer metastasis .
	manualset3
266819	3	426732	16	NULL	NULL	NULL	NULL	epithelial-mesenchymal transition ( EMT )	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E-cadherin is a hallmark of epithelial-mesenchymal transition ( EMT ) , which plays a crucial role in cancer metastasis .
	manualset3
266820	4	426732	16	NULL	NULL	NULL	NULL	role	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E-cadherin is a hallmark of epithelial-mesenchymal transition ( EMT ) , which plays a crucial role in cancer metastasis .
	manualset3
266821	5	426732	16	NULL	NULL	NULL	NULL	cancer metastasis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E-cadherin is a hallmark of epithelial-mesenchymal transition ( EMT ) , which plays a crucial role in cancer metastasis .
	manualset3
266822	1	426733	16	NULL	NULL	NULL	NULL	E. coli CN1016	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E. coli CN1016 had reduced survival and inflammatogenicity in the mouse urinary tract infection model .
	manualset3
266823	2	426733	16	NULL	NULL	NULL	NULL	reduced survival	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E. coli CN1016 had reduced survival and inflammatogenicity in the mouse urinary tract infection model .
	manualset3
266824	3	426733	16	NULL	NULL	NULL	NULL	mouse urinary tract infection model	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E. coli CN1016 had reduced survival and inflammatogenicity in the mouse urinary tract infection model .
	manualset3
266825	1	426734	16	NULL	NULL	NULL	NULL	E. coli	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E. coli was sensible to the TSU in 54.4 % of cases .
	manualset3
266826	2	426734	16	NULL	NULL	NULL	NULL	TSU	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E. coli was sensible to the TSU in 54.4 % of cases .
	manualset3
266827	3	426734	16	NULL	NULL	NULL	NULL	54.4 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E. coli was sensible to the TSU in 54.4 % of cases .
	manualset3
266828	4	426734	16	NULL	NULL	NULL	NULL	cases	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E. coli was sensible to the TSU in 54.4 % of cases .
	manualset3
266829	1	426735	16	NULL	NULL	NULL	NULL	E ( 2 )	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E ( 2 ) reduced food intake , body weight , and visceral fat content in both Ovx-DS/obese and Ovx-DS/lean rats .
	manualset3
266830	2	426735	16	NULL	NULL	NULL	NULL	food intake	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E ( 2 ) reduced food intake , body weight , and visceral fat content in both Ovx-DS/obese and Ovx-DS/lean rats .
	manualset3
266831	3	426735	16	NULL	NULL	NULL	NULL	body weight	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E ( 2 ) reduced food intake , body weight , and visceral fat content in both Ovx-DS/obese and Ovx-DS/lean rats .
	manualset3
266832	4	426735	16	NULL	NULL	NULL	NULL	visceral fat content	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E ( 2 ) reduced food intake , body weight , and visceral fat content in both Ovx-DS/obese and Ovx-DS/lean rats .
	manualset3
266833	5	426735	16	NULL	NULL	NULL	NULL	Ovx-DS/obese rats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E ( 2 ) reduced food intake , body weight , and visceral fat content in both Ovx-DS/obese and Ovx-DS/lean rats .
	manualset3
266834	6	426735	16	NULL	NULL	NULL	NULL	Ovx-DS/lean rats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	E ( 2 ) reduced food intake , body weight , and visceral fat content in both Ovx-DS/obese and Ovx-DS/lean rats .
	manualset3
266835	1	426736	16	NULL	NULL	NULL	NULL	EA	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EA did not affect basal Mn-SOD activity and inhibited IL-1 beta-stimulated activity , whereas EA-S was without effect .
	manualset3
266836	2	426736	16	NULL	NULL	NULL	NULL	Mn-SOD activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EA did not affect basal Mn-SOD activity and inhibited IL-1 beta-stimulated activity , whereas EA-S was without effect .
	manualset3
266837	3	426736	16	NULL	NULL	NULL	NULL	IL-1 beta-stimulated activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EA did not affect basal Mn-SOD activity and inhibited IL-1 beta-stimulated activity , whereas EA-S was without effect .
	manualset3
266838	4	426736	16	NULL	NULL	NULL	NULL	EA-S	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EA did not affect basal Mn-SOD activity and inhibited IL-1 beta-stimulated activity , whereas EA-S was without effect .
	manualset3
266839	5	426736	16	NULL	NULL	NULL	NULL	effect	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EA did not affect basal Mn-SOD activity and inhibited IL-1 beta-stimulated activity , whereas EA-S was without effect .
	manualset3
266840	1	426737	16	NULL	NULL	NULL	NULL	EBp	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EBp is 24-fold more toxic ( LD50 = 91 + / - 14 mg/kg body wt ) than Bp ( LD50 = 2218 + / - 195 mg/kg body wt ) and only EBp produced characteristic tremors and lacrimation .
	manualset3
266841	2	426737	16	NULL	NULL	NULL	NULL	24-fold	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EBp is 24-fold more toxic ( LD50 = 91 + / - 14 mg/kg body wt ) than Bp ( LD50 = 2218 + / - 195 mg/kg body wt ) and only EBp produced characteristic tremors and lacrimation .
	manualset3
266842	3	426737	16	NULL	NULL	NULL	NULL	LD50 = 91 + / - 14 mg/kg body wt	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EBp is 24-fold more toxic ( LD50 = 91 + / - 14 mg/kg body wt ) than Bp ( LD50 = 2218 + / - 195 mg/kg body wt ) and only EBp produced characteristic tremors and lacrimation .
	manualset3
266843	4	426737	16	NULL	NULL	NULL	NULL	Bp	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EBp is 24-fold more toxic ( LD50 = 91 + / - 14 mg/kg body wt ) than Bp ( LD50 = 2218 + / - 195 mg/kg body wt ) and only EBp produced characteristic tremors and lacrimation .
	manualset3
266844	5	426737	16	NULL	NULL	NULL	NULL	LD50 = 2218 + / - 195 mg/kg body wt	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EBp is 24-fold more toxic ( LD50 = 91 + / - 14 mg/kg body wt ) than Bp ( LD50 = 2218 + / - 195 mg/kg body wt ) and only EBp produced characteristic tremors and lacrimation .
	manualset3
266845	6	426737	16	NULL	NULL	NULL	NULL	EBp	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EBp is 24-fold more toxic ( LD50 = 91 + / - 14 mg/kg body wt ) than Bp ( LD50 = 2218 + / - 195 mg/kg body wt ) and only EBp produced characteristic tremors and lacrimation .
	manualset3
266846	7	426737	16	NULL	NULL	NULL	NULL	characteristic tremors	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EBp is 24-fold more toxic ( LD50 = 91 + / - 14 mg/kg body wt ) than Bp ( LD50 = 2218 + / - 195 mg/kg body wt ) and only EBp produced characteristic tremors and lacrimation .
	manualset3
266847	8	426737	16	NULL	NULL	NULL	NULL	lacrimation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EBp is 24-fold more toxic ( LD50 = 91 + / - 14 mg/kg body wt ) than Bp ( LD50 = 2218 + / - 195 mg/kg body wt ) and only EBp produced characteristic tremors and lacrimation .
	manualset3
266848	1	426738	16	NULL	NULL	NULL	NULL	EC migration	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EC migration ( 90.7 % + / - 6.2 % : p = ns ) was not inhibited by 0.1 mg/ml of coacervated alpha-elastin .
	manualset3
266849	2	426738	16	NULL	NULL	NULL	NULL	90.7 % + / - 6.2 % : p = ns	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EC migration ( 90.7 % + / - 6.2 % : p = ns ) was not inhibited by 0.1 mg/ml of coacervated alpha-elastin .
	manualset3
266850	3	426738	16	NULL	NULL	NULL	NULL	0.1 mg/ml	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EC migration ( 90.7 % + / - 6.2 % : p = ns ) was not inhibited by 0.1 mg/ml of coacervated alpha-elastin .
	manualset3
266851	4	426738	16	NULL	NULL	NULL	NULL	coacervated alpha-elastin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EC migration ( 90.7 % + / - 6.2 % : p = ns ) was not inhibited by 0.1 mg/ml of coacervated alpha-elastin .
	manualset3
266852	1	426739	16	NULL	NULL	NULL	NULL	EC movements	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EC movements on fibronectin and interstitial collagens were similar ( X velocity = 0.2 micron/min ) .
	manualset3
266853	2	426739	16	NULL	NULL	NULL	NULL	fibronectin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EC movements on fibronectin and interstitial collagens were similar ( X velocity = 0.2 micron/min ) .
	manualset3
266854	3	426739	16	NULL	NULL	NULL	NULL	interstitial collagens	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EC movements on fibronectin and interstitial collagens were similar ( X velocity = 0.2 micron/min ) .
	manualset3
266855	4	426739	16	NULL	NULL	NULL	NULL	X velocity	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EC movements on fibronectin and interstitial collagens were similar ( X velocity = 0.2 micron/min ) .
	manualset3
266856	5	426739	16	NULL	NULL	NULL	NULL	0.2 micron/min	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EC movements on fibronectin and interstitial collagens were similar ( X velocity = 0.2 micron/min ) .
	manualset3
266857	1	426740	16	NULL	NULL	NULL	NULL	ECS	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ECS given daily for five consecutive days increased CART mRNA and protein in the rat nucleus accumbens ( NAc ) , accompanied by an increase in CREB phosphorylation .
	manualset3
266858	2	426740	16	NULL	NULL	NULL	NULL	five consecutive days	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ECS given daily for five consecutive days increased CART mRNA and protein in the rat nucleus accumbens ( NAc ) , accompanied by an increase in CREB phosphorylation .
	manualset3
266859	3	426740	16	NULL	NULL	NULL	NULL	CART mRNA	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ECS given daily for five consecutive days increased CART mRNA and protein in the rat nucleus accumbens ( NAc ) , accompanied by an increase in CREB phosphorylation .
	manualset3
266860	4	426740	16	NULL	NULL	NULL	NULL	CART protein	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ECS given daily for five consecutive days increased CART mRNA and protein in the rat nucleus accumbens ( NAc ) , accompanied by an increase in CREB phosphorylation .
	manualset3
266861	5	426740	16	NULL	NULL	NULL	NULL	rat	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ECS given daily for five consecutive days increased CART mRNA and protein in the rat nucleus accumbens ( NAc ) , accompanied by an increase in CREB phosphorylation .
	manualset3
266862	6	426740	16	NULL	NULL	NULL	NULL	nucleus accumbens ( NAc )	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ECS given daily for five consecutive days increased CART mRNA and protein in the rat nucleus accumbens ( NAc ) , accompanied by an increase in CREB phosphorylation .
	manualset3
266863	7	426740	16	NULL	NULL	NULL	NULL	increase	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ECS given daily for five consecutive days increased CART mRNA and protein in the rat nucleus accumbens ( NAc ) , accompanied by an increase in CREB phosphorylation .
	manualset3
266864	8	426740	16	NULL	NULL	NULL	NULL	CREB phosphorylation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ECS given daily for five consecutive days increased CART mRNA and protein in the rat nucleus accumbens ( NAc ) , accompanied by an increase in CREB phosphorylation .
	manualset3
266865	1	426741	16	NULL	NULL	NULL	NULL	ECT	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ECT was found to be an effective treatment procedure in mood disorders .
	manualset3
266866	2	426741	16	NULL	NULL	NULL	NULL	effective treatment procedure	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ECT was found to be an effective treatment procedure in mood disorders .
	manualset3
266867	3	426741	16	NULL	NULL	NULL	NULL	mood disorders	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ECT was found to be an effective treatment procedure in mood disorders .
	manualset3
266868	1	426742	16	NULL	NULL	NULL	NULL	EDHF	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EDHF relaxes vascular smooth muscle through activation of ATP-dependent potassium channels .
	manualset3
266869	2	426742	16	NULL	NULL	NULL	NULL	vascular smooth muscle	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EDHF relaxes vascular smooth muscle through activation of ATP-dependent potassium channels .
	manualset3
266870	3	426742	16	NULL	NULL	NULL	NULL	activation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EDHF relaxes vascular smooth muscle through activation of ATP-dependent potassium channels .
	manualset3
266871	4	426742	16	NULL	NULL	NULL	NULL	ATP-dependent potassium channels	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EDHF relaxes vascular smooth muscle through activation of ATP-dependent potassium channels .
	manualset3
266872	1	426743	16	NULL	NULL	NULL	NULL	EDTA	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EDTA bleaching was observed only in intact leaves .
	manualset3
266873	2	426743	16	NULL	NULL	NULL	NULL	intact leaves	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EDTA bleaching was observed only in intact leaves .
	manualset3
266874	1	426744	16	NULL	NULL	NULL	NULL	EFA supplementation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EFA supplementation ( evening primrose oil ; Efamol ) resulted in significantly lower levels of palmitoleic acid ( a nonessential fatty acid ) and higher concentrations of dihomogammalinolenic acid , an EFA previously found to be deficient in some hyperactive children .
	manualset3
266875	2	426744	16	NULL	NULL	NULL	NULL	evening primrose oil	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EFA supplementation ( evening primrose oil ; Efamol ) resulted in significantly lower levels of palmitoleic acid ( a nonessential fatty acid ) and higher concentrations of dihomogammalinolenic acid , an EFA previously found to be deficient in some hyperactive children .
	manualset3
266876	3	426744	16	NULL	NULL	NULL	NULL	Efamol	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EFA supplementation ( evening primrose oil ; Efamol ) resulted in significantly lower levels of palmitoleic acid ( a nonessential fatty acid ) and higher concentrations of dihomogammalinolenic acid , an EFA previously found to be deficient in some hyperactive children .
	manualset3
266877	4	426744	16	NULL	NULL	NULL	NULL	levels	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EFA supplementation ( evening primrose oil ; Efamol ) resulted in significantly lower levels of palmitoleic acid ( a nonessential fatty acid ) and higher concentrations of dihomogammalinolenic acid , an EFA previously found to be deficient in some hyperactive children .
	manualset3
266878	5	426744	16	NULL	NULL	NULL	NULL	palmitoleic acid	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EFA supplementation ( evening primrose oil ; Efamol ) resulted in significantly lower levels of palmitoleic acid ( a nonessential fatty acid ) and higher concentrations of dihomogammalinolenic acid , an EFA previously found to be deficient in some hyperactive children .
	manualset3
266879	6	426744	16	NULL	NULL	NULL	NULL	nonessential fatty acid	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EFA supplementation ( evening primrose oil ; Efamol ) resulted in significantly lower levels of palmitoleic acid ( a nonessential fatty acid ) and higher concentrations of dihomogammalinolenic acid , an EFA previously found to be deficient in some hyperactive children .
	manualset3
266880	7	426744	16	NULL	NULL	NULL	NULL	concentrations	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EFA supplementation ( evening primrose oil ; Efamol ) resulted in significantly lower levels of palmitoleic acid ( a nonessential fatty acid ) and higher concentrations of dihomogammalinolenic acid , an EFA previously found to be deficient in some hyperactive children .
	manualset3
266881	8	426744	16	NULL	NULL	NULL	NULL	dihomogammalinolenic acid	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EFA supplementation ( evening primrose oil ; Efamol ) resulted in significantly lower levels of palmitoleic acid ( a nonessential fatty acid ) and higher concentrations of dihomogammalinolenic acid , an EFA previously found to be deficient in some hyperactive children .
	manualset3
266882	9	426744	16	NULL	NULL	NULL	NULL	EFA	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EFA supplementation ( evening primrose oil ; Efamol ) resulted in significantly lower levels of palmitoleic acid ( a nonessential fatty acid ) and higher concentrations of dihomogammalinolenic acid , an EFA previously found to be deficient in some hyperactive children .
	manualset3
266883	10	426744	16	NULL	NULL	NULL	NULL	hyperactive children	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EFA supplementation ( evening primrose oil ; Efamol ) resulted in significantly lower levels of palmitoleic acid ( a nonessential fatty acid ) and higher concentrations of dihomogammalinolenic acid , an EFA previously found to be deficient in some hyperactive children .
	manualset3
266884	1	426745	16	NULL	NULL	NULL	NULL	EGCG	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EGCG added to a liposome dispersion existed either in a buffer solution as aggregates or in phospholipid bilayer membranes , and EGCG disturbed membrane structure .
	manualset3
266885	2	426745	16	NULL	NULL	NULL	NULL	liposome dispersion	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EGCG added to a liposome dispersion existed either in a buffer solution as aggregates or in phospholipid bilayer membranes , and EGCG disturbed membrane structure .
	manualset3
266886	3	426745	16	NULL	NULL	NULL	NULL	buffer solution	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EGCG added to a liposome dispersion existed either in a buffer solution as aggregates or in phospholipid bilayer membranes , and EGCG disturbed membrane structure .
	manualset3
266887	4	426745	16	NULL	NULL	NULL	NULL	aggregates	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EGCG added to a liposome dispersion existed either in a buffer solution as aggregates or in phospholipid bilayer membranes , and EGCG disturbed membrane structure .
	manualset3
266888	5	426745	16	NULL	NULL	NULL	NULL	phospholipid bilayer membranes	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EGCG added to a liposome dispersion existed either in a buffer solution as aggregates or in phospholipid bilayer membranes , and EGCG disturbed membrane structure .
	manualset3
266889	6	426745	16	NULL	NULL	NULL	NULL	EGCG	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EGCG added to a liposome dispersion existed either in a buffer solution as aggregates or in phospholipid bilayer membranes , and EGCG disturbed membrane structure .
	manualset3
266890	7	426745	16	NULL	NULL	NULL	NULL	membrane structure	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EGCG added to a liposome dispersion existed either in a buffer solution as aggregates or in phospholipid bilayer membranes , and EGCG disturbed membrane structure .
	manualset3
266891	1	426746	16	NULL	NULL	NULL	NULL	EGF-stimulated uptake	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EGF-stimulated uptake appeared to be due predominantly to the cotransporter .
	manualset3
266892	2	426746	16	NULL	NULL	NULL	NULL	cotransporter	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EGF-stimulated uptake appeared to be due predominantly to the cotransporter .
	manualset3
266893	1	426747	16	NULL	NULL	NULL	NULL	 Abdominal-pelvic actinomycosis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Abdominal-pelvic actinomycosis with urinary tract involvement , secondary to gynecologic infection caused by intrauterine device ) .
	manualset3
266894	2	426747	16	NULL	NULL	NULL	NULL	urinary tract involvement	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Abdominal-pelvic actinomycosis with urinary tract involvement , secondary to gynecologic infection caused by intrauterine device ) .
	manualset3
266895	3	426747	16	NULL	NULL	NULL	NULL	gynecologic infection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Abdominal-pelvic actinomycosis with urinary tract involvement , secondary to gynecologic infection caused by intrauterine device ) .
	manualset3
266896	4	426747	16	NULL	NULL	NULL	NULL	intrauterine device	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Abdominal-pelvic actinomycosis with urinary tract involvement , secondary to gynecologic infection caused by intrauterine device ) .
	manualset3
266897	1	426748	16	NULL	NULL	NULL	NULL	EGF-treatment	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EGF-treatment-induced transient impairment in tyrosine hydroxylase expression .
	manualset3
266898	2	426748	16	NULL	NULL	NULL	NULL	transient impairment	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EGF-treatment-induced transient impairment in tyrosine hydroxylase expression .
	manualset3
266899	3	426748	16	NULL	NULL	NULL	NULL	tyrosine hydroxylase expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EGF-treatment-induced transient impairment in tyrosine hydroxylase expression .
	manualset3
266900	1	426749	16	NULL	NULL	NULL	NULL	EGF	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EGF has also got a suppressive effect on 17 a-hydroxylase enzyme ; a key enzyme which is necessary for the hydroxylation of pregnenolone and progesterone in the ovary Hydroxy pregnenolone is a precursor of androstendione , while 17 a-hydroxyprogesterone is a precursor of testosterone .
	manualset3
266901	2	426749	16	NULL	NULL	NULL	NULL	suppressive effect	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EGF has also got a suppressive effect on 17 a-hydroxylase enzyme ; a key enzyme which is necessary for the hydroxylation of pregnenolone and progesterone in the ovary Hydroxy pregnenolone is a precursor of androstendione , while 17 a-hydroxyprogesterone is a precursor of testosterone .
	manualset3
266902	3	426749	16	NULL	NULL	NULL	NULL	17 a-hydroxylase enzyme	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EGF has also got a suppressive effect on 17 a-hydroxylase enzyme ; a key enzyme which is necessary for the hydroxylation of pregnenolone and progesterone in the ovary Hydroxy pregnenolone is a precursor of androstendione , while 17 a-hydroxyprogesterone is a precursor of testosterone .
	manualset3
266903	4	426749	16	NULL	NULL	NULL	NULL	enzyme	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EGF has also got a suppressive effect on 17 a-hydroxylase enzyme ; a key enzyme which is necessary for the hydroxylation of pregnenolone and progesterone in the ovary Hydroxy pregnenolone is a precursor of androstendione , while 17 a-hydroxyprogesterone is a precursor of testosterone .
	manualset3
266904	5	426749	16	NULL	NULL	NULL	NULL	hydroxylation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EGF has also got a suppressive effect on 17 a-hydroxylase enzyme ; a key enzyme which is necessary for the hydroxylation of pregnenolone and progesterone in the ovary Hydroxy pregnenolone is a precursor of androstendione , while 17 a-hydroxyprogesterone is a precursor of testosterone .
	manualset3
266905	6	426749	16	NULL	NULL	NULL	NULL	pregnenolone	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EGF has also got a suppressive effect on 17 a-hydroxylase enzyme ; a key enzyme which is necessary for the hydroxylation of pregnenolone and progesterone in the ovary Hydroxy pregnenolone is a precursor of androstendione , while 17 a-hydroxyprogesterone is a precursor of testosterone .
	manualset3
266906	7	426749	16	NULL	NULL	NULL	NULL	progesterone	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EGF has also got a suppressive effect on 17 a-hydroxylase enzyme ; a key enzyme which is necessary for the hydroxylation of pregnenolone and progesterone in the ovary Hydroxy pregnenolone is a precursor of androstendione , while 17 a-hydroxyprogesterone is a precursor of testosterone .
	manualset3
266907	8	426749	16	NULL	NULL	NULL	NULL	ovary	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EGF has also got a suppressive effect on 17 a-hydroxylase enzyme ; a key enzyme which is necessary for the hydroxylation of pregnenolone and progesterone in the ovary Hydroxy pregnenolone is a precursor of androstendione , while 17 a-hydroxyprogesterone is a precursor of testosterone .
	manualset3
266908	9	426749	16	NULL	NULL	NULL	NULL	Hydroxy pregnenolone	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EGF has also got a suppressive effect on 17 a-hydroxylase enzyme ; a key enzyme which is necessary for the hydroxylation of pregnenolone and progesterone in the ovary Hydroxy pregnenolone is a precursor of androstendione , while 17 a-hydroxyprogesterone is a precursor of testosterone .
	manualset3
266909	10	426749	16	NULL	NULL	NULL	NULL	precursor	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EGF has also got a suppressive effect on 17 a-hydroxylase enzyme ; a key enzyme which is necessary for the hydroxylation of pregnenolone and progesterone in the ovary Hydroxy pregnenolone is a precursor of androstendione , while 17 a-hydroxyprogesterone is a precursor of testosterone .
	manualset3
266910	11	426749	16	NULL	NULL	NULL	NULL	androstendione	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EGF has also got a suppressive effect on 17 a-hydroxylase enzyme ; a key enzyme which is necessary for the hydroxylation of pregnenolone and progesterone in the ovary Hydroxy pregnenolone is a precursor of androstendione , while 17 a-hydroxyprogesterone is a precursor of testosterone .
	manualset3
266911	12	426749	16	NULL	NULL	NULL	NULL	17 a-hydroxyprogesterone	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EGF has also got a suppressive effect on 17 a-hydroxylase enzyme ; a key enzyme which is necessary for the hydroxylation of pregnenolone and progesterone in the ovary Hydroxy pregnenolone is a precursor of androstendione , while 17 a-hydroxyprogesterone is a precursor of testosterone .
	manualset3
266912	13	426749	16	NULL	NULL	NULL	NULL	precursor	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EGF has also got a suppressive effect on 17 a-hydroxylase enzyme ; a key enzyme which is necessary for the hydroxylation of pregnenolone and progesterone in the ovary Hydroxy pregnenolone is a precursor of androstendione , while 17 a-hydroxyprogesterone is a precursor of testosterone .
	manualset3
266913	14	426749	16	NULL	NULL	NULL	NULL	testosterone	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EGF has also got a suppressive effect on 17 a-hydroxylase enzyme ; a key enzyme which is necessary for the hydroxylation of pregnenolone and progesterone in the ovary Hydroxy pregnenolone is a precursor of androstendione , while 17 a-hydroxyprogesterone is a precursor of testosterone .
	manualset3
266922	1	426751	16	NULL	NULL	NULL	NULL	ELISA	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ELISA was used to screen plasma samples for antibodies to HTLV-I , and the positive samples were tested by a confirmatory assay ( Western blotting ) .
	manualset3
266923	2	426751	16	NULL	NULL	NULL	NULL	plasma samples	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ELISA was used to screen plasma samples for antibodies to HTLV-I , and the positive samples were tested by a confirmatory assay ( Western blotting ) .
	manualset3
266924	3	426751	16	NULL	NULL	NULL	NULL	antibodies	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ELISA was used to screen plasma samples for antibodies to HTLV-I , and the positive samples were tested by a confirmatory assay ( Western blotting ) .
	manualset3
266925	4	426751	16	NULL	NULL	NULL	NULL	HTLV-I	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ELISA was used to screen plasma samples for antibodies to HTLV-I , and the positive samples were tested by a confirmatory assay ( Western blotting ) .
	manualset3
266926	5	426751	16	NULL	NULL	NULL	NULL	positive samples	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ELISA was used to screen plasma samples for antibodies to HTLV-I , and the positive samples were tested by a confirmatory assay ( Western blotting ) .
	manualset3
266927	6	426751	16	NULL	NULL	NULL	NULL	confirmatory assay	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ELISA was used to screen plasma samples for antibodies to HTLV-I , and the positive samples were tested by a confirmatory assay ( Western blotting ) .
	manualset3
266928	7	426751	16	NULL	NULL	NULL	NULL	Western blotting	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ELISA was used to screen plasma samples for antibodies to HTLV-I , and the positive samples were tested by a confirmatory assay ( Western blotting ) .
	manualset3
266929	1	426752	16	NULL	NULL	NULL	NULL	EMMPRIN ( CD147 , extracellular matrix metalloproteinase inducer )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EMMPRIN ( CD147 , extracellular matrix metalloproteinase inducer ) is a cell surface protein that is expressed among other cell types , in particular in tumor cells .
	manualset3
266930	2	426752	16	NULL	NULL	NULL	NULL	cell surface protein	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EMMPRIN ( CD147 , extracellular matrix metalloproteinase inducer ) is a cell surface protein that is expressed among other cell types , in particular in tumor cells .
	manualset3
266931	3	426752	16	NULL	NULL	NULL	NULL	cell types	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EMMPRIN ( CD147 , extracellular matrix metalloproteinase inducer ) is a cell surface protein that is expressed among other cell types , in particular in tumor cells .
	manualset3
266932	4	426752	16	NULL	NULL	NULL	NULL	tumor cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EMMPRIN ( CD147 , extracellular matrix metalloproteinase inducer ) is a cell surface protein that is expressed among other cell types , in particular in tumor cells .
	manualset3
266933	1	426753	16	NULL	NULL	NULL	NULL	ENI	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ENI and SNI both created a dose gradient to the lymph nodes across the mediastinum .
	manualset3
266934	2	426753	16	NULL	NULL	NULL	NULL	SNI	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ENI and SNI both created a dose gradient to the lymph nodes across the mediastinum .
	manualset3
266935	3	426753	16	NULL	NULL	NULL	NULL	dose gradient	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ENI and SNI both created a dose gradient to the lymph nodes across the mediastinum .
	manualset3
266936	4	426753	16	NULL	NULL	NULL	NULL	lymph nodes	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ENI and SNI both created a dose gradient to the lymph nodes across the mediastinum .
	manualset3
266937	5	426753	16	NULL	NULL	NULL	NULL	mediastinum	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ENI and SNI both created a dose gradient to the lymph nodes across the mediastinum .
	manualset3
266938	1	426754	16	NULL	NULL	NULL	NULL	ENU mouse mutagenesis programs	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ENU mouse mutagenesis programs will enable advances in the diagnosis and treatment of human male infertility and ultimately aid in the development of novel male-based contraceptives .
	manualset3
266939	2	426754	16	NULL	NULL	NULL	NULL	advances	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ENU mouse mutagenesis programs will enable advances in the diagnosis and treatment of human male infertility and ultimately aid in the development of novel male-based contraceptives .
	manualset3
266940	3	426754	16	NULL	NULL	NULL	NULL	diagnosis	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ENU mouse mutagenesis programs will enable advances in the diagnosis and treatment of human male infertility and ultimately aid in the development of novel male-based contraceptives .
	manualset3
266941	4	426754	16	NULL	NULL	NULL	NULL	treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ENU mouse mutagenesis programs will enable advances in the diagnosis and treatment of human male infertility and ultimately aid in the development of novel male-based contraceptives .
	manualset3
266942	5	426754	16	NULL	NULL	NULL	NULL	human male infertility	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ENU mouse mutagenesis programs will enable advances in the diagnosis and treatment of human male infertility and ultimately aid in the development of novel male-based contraceptives .
	manualset3
266943	6	426754	16	NULL	NULL	NULL	NULL	development	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ENU mouse mutagenesis programs will enable advances in the diagnosis and treatment of human male infertility and ultimately aid in the development of novel male-based contraceptives .
	manualset3
266944	7	426754	16	NULL	NULL	NULL	NULL	male-based contraceptives	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ENU mouse mutagenesis programs will enable advances in the diagnosis and treatment of human male infertility and ultimately aid in the development of novel male-based contraceptives .
	manualset3
266945	1	426755	16	NULL	NULL	NULL	NULL	ENU mutagenesis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ENU mutagenesis : analyzing gene function in mice .
	manualset3
266946	2	426755	16	NULL	NULL	NULL	NULL	gene function	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ENU mutagenesis : analyzing gene function in mice .
	manualset3
266947	3	426755	16	NULL	NULL	NULL	NULL	mice	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ENU mutagenesis : analyzing gene function in mice .
	manualset3
266948	1	426756	16	NULL	NULL	NULL	NULL	EPR analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EPR analysis indicates that ethanedithiolate ( 2 ) ( + ) exists as a single species at 110 K , whereas the propanedithiolate cations exist as a mixture of two conformers , which are proposed to be related through a flip of the chelate ring .
	manualset3
266949	2	426756	16	NULL	NULL	NULL	NULL	ethanedithiolate ( 2 ) ( + )	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EPR analysis indicates that ethanedithiolate ( 2 ) ( + ) exists as a single species at 110 K , whereas the propanedithiolate cations exist as a mixture of two conformers , which are proposed to be related through a flip of the chelate ring .
	manualset3
266950	3	426756	16	NULL	NULL	NULL	NULL	single species	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EPR analysis indicates that ethanedithiolate ( 2 ) ( + ) exists as a single species at 110 K , whereas the propanedithiolate cations exist as a mixture of two conformers , which are proposed to be related through a flip of the chelate ring .
	manualset3
266951	4	426756	16	NULL	NULL	NULL	NULL	110 K	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EPR analysis indicates that ethanedithiolate ( 2 ) ( + ) exists as a single species at 110 K , whereas the propanedithiolate cations exist as a mixture of two conformers , which are proposed to be related through a flip of the chelate ring .
	manualset3
266952	5	426756	16	NULL	NULL	NULL	NULL	propanedithiolate cations	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EPR analysis indicates that ethanedithiolate ( 2 ) ( + ) exists as a single species at 110 K , whereas the propanedithiolate cations exist as a mixture of two conformers , which are proposed to be related through a flip of the chelate ring .
	manualset3
266953	6	426756	16	NULL	NULL	NULL	NULL	mixture	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EPR analysis indicates that ethanedithiolate ( 2 ) ( + ) exists as a single species at 110 K , whereas the propanedithiolate cations exist as a mixture of two conformers , which are proposed to be related through a flip of the chelate ring .
	manualset3
266954	7	426756	16	NULL	NULL	NULL	NULL	two conformers	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EPR analysis indicates that ethanedithiolate ( 2 ) ( + ) exists as a single species at 110 K , whereas the propanedithiolate cations exist as a mixture of two conformers , which are proposed to be related through a flip of the chelate ring .
	manualset3
266955	8	426756	16	NULL	NULL	NULL	NULL	flip	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EPR analysis indicates that ethanedithiolate ( 2 ) ( + ) exists as a single species at 110 K , whereas the propanedithiolate cations exist as a mixture of two conformers , which are proposed to be related through a flip of the chelate ring .
	manualset3
266956	9	426756	16	NULL	NULL	NULL	NULL	chelate ring	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EPR analysis indicates that ethanedithiolate ( 2 ) ( + ) exists as a single species at 110 K , whereas the propanedithiolate cations exist as a mixture of two conformers , which are proposed to be related through a flip of the chelate ring .
	manualset3
266957	1	426757	16	NULL	NULL	NULL	NULL	ERBB2 genes	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERBB2 genes but not TOP2A genes are present in tandem amplicons , leading to a higher ERBB2 ratio .
	manualset3
266958	2	426757	16	NULL	NULL	NULL	NULL	TOP2A genes	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERBB2 genes but not TOP2A genes are present in tandem amplicons , leading to a higher ERBB2 ratio .
	manualset3
266959	3	426757	16	NULL	NULL	NULL	NULL	tandem amplicons	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERBB2 genes but not TOP2A genes are present in tandem amplicons , leading to a higher ERBB2 ratio .
	manualset3
266960	4	426757	16	NULL	NULL	NULL	NULL	higher ERBB2 ratio	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERBB2 genes but not TOP2A genes are present in tandem amplicons , leading to a higher ERBB2 ratio .
	manualset3
266961	1	426758	16	NULL	NULL	NULL	NULL	ERH depletion	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERH depletion also caused dissociation of centromere-associated protein E ( CENP-E ) , a mitotic kinesin that is involved in stabilizing the kinetochore-microtubule attachment , from kinetochores of mitotic chromosomes .
	manualset3
266962	2	426758	16	NULL	NULL	NULL	NULL	dissociation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERH depletion also caused dissociation of centromere-associated protein E ( CENP-E ) , a mitotic kinesin that is involved in stabilizing the kinetochore-microtubule attachment , from kinetochores of mitotic chromosomes .
	manualset3
266963	3	426758	16	NULL	NULL	NULL	NULL	centromere-associated protein E ( CENP-E )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERH depletion also caused dissociation of centromere-associated protein E ( CENP-E ) , a mitotic kinesin that is involved in stabilizing the kinetochore-microtubule attachment , from kinetochores of mitotic chromosomes .
	manualset3
266964	4	426758	16	NULL	NULL	NULL	NULL	mitotic kinesin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERH depletion also caused dissociation of centromere-associated protein E ( CENP-E ) , a mitotic kinesin that is involved in stabilizing the kinetochore-microtubule attachment , from kinetochores of mitotic chromosomes .
	manualset3
266965	5	426758	16	NULL	NULL	NULL	NULL	 kinetochore-microtubule attachment	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERH depletion also caused dissociation of centromere-associated protein E ( CENP-E ) , a mitotic kinesin that is involved in stabilizing the kinetochore-microtubule attachment , from kinetochores of mitotic chromosomes .
	manualset3
266966	6	426758	16	NULL	NULL	NULL	NULL	kinetochores	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERH depletion also caused dissociation of centromere-associated protein E ( CENP-E ) , a mitotic kinesin that is involved in stabilizing the kinetochore-microtubule attachment , from kinetochores of mitotic chromosomes .
	manualset3
266967	7	426758	16	NULL	NULL	NULL	NULL	mitotic chromosomes	Chromosome												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERH depletion also caused dissociation of centromere-associated protein E ( CENP-E ) , a mitotic kinesin that is involved in stabilizing the kinetochore-microtubule attachment , from kinetochores of mitotic chromosomes .
	manualset3
266968	1	426759	16	NULL	NULL	NULL	NULL	ERK1/2 pathways	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERK1/2 and JNK pathways are involved in this bipartite response , which can lead to neurodegeneration or neuroprotection depending on the cellular and environmental conditions or cooperation with other signalling pathways such as Akt cascade .
	manualset3
266969	2	426759	16	NULL	NULL	NULL	NULL	JNK pathways	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERK1/2 and JNK pathways are involved in this bipartite response , which can lead to neurodegeneration or neuroprotection depending on the cellular and environmental conditions or cooperation with other signalling pathways such as Akt cascade .
	manualset3
266970	3	426759	16	NULL	NULL	NULL	NULL	bipartite response	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERK1/2 and JNK pathways are involved in this bipartite response , which can lead to neurodegeneration or neuroprotection depending on the cellular and environmental conditions or cooperation with other signalling pathways such as Akt cascade .
	manualset3
266971	4	426759	16	NULL	NULL	NULL	NULL	neurodegeneration	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERK1/2 and JNK pathways are involved in this bipartite response , which can lead to neurodegeneration or neuroprotection depending on the cellular and environmental conditions or cooperation with other signalling pathways such as Akt cascade .
	manualset3
266972	5	426759	16	NULL	NULL	NULL	NULL	neuroprotection	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERK1/2 and JNK pathways are involved in this bipartite response , which can lead to neurodegeneration or neuroprotection depending on the cellular and environmental conditions or cooperation with other signalling pathways such as Akt cascade .
	manualset3
266973	6	426759	16	NULL	NULL	NULL	NULL	cellular conditions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERK1/2 and JNK pathways are involved in this bipartite response , which can lead to neurodegeneration or neuroprotection depending on the cellular and environmental conditions or cooperation with other signalling pathways such as Akt cascade .
	manualset3
266974	7	426759	16	NULL	NULL	NULL	NULL	environmental conditions	EnvironmentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERK1/2 and JNK pathways are involved in this bipartite response , which can lead to neurodegeneration or neuroprotection depending on the cellular and environmental conditions or cooperation with other signalling pathways such as Akt cascade .
	manualset3
266975	8	426759	16	NULL	NULL	NULL	NULL	cooperation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERK1/2 and JNK pathways are involved in this bipartite response , which can lead to neurodegeneration or neuroprotection depending on the cellular and environmental conditions or cooperation with other signalling pathways such as Akt cascade .
	manualset3
266976	9	426759	16	NULL	NULL	NULL	NULL	signalling pathways	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERK1/2 and JNK pathways are involved in this bipartite response , which can lead to neurodegeneration or neuroprotection depending on the cellular and environmental conditions or cooperation with other signalling pathways such as Akt cascade .
	manualset3
266977	10	426759	16	NULL	NULL	NULL	NULL	Akt cascade	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERK1/2 and JNK pathways are involved in this bipartite response , which can lead to neurodegeneration or neuroprotection depending on the cellular and environmental conditions or cooperation with other signalling pathways such as Akt cascade .
	manualset3
266978	1	426760	16	NULL	NULL	NULL	NULL	ERPF	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERPF , ERBF , and GFR were lower in patients homozygous for the 460Trp allele compared with patients with the Gly460Gly genotype on low sodium diet but no differences were found at the higher sodium intake .
	manualset3
266979	2	426760	16	NULL	NULL	NULL	NULL	ERBF	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERPF , ERBF , and GFR were lower in patients homozygous for the 460Trp allele compared with patients with the Gly460Gly genotype on low sodium diet but no differences were found at the higher sodium intake .
	manualset3
266980	3	426760	16	NULL	NULL	NULL	NULL	GFR	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERPF , ERBF , and GFR were lower in patients homozygous for the 460Trp allele compared with patients with the Gly460Gly genotype on low sodium diet but no differences were found at the higher sodium intake .
	manualset3
266981	4	426760	16	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERPF , ERBF , and GFR were lower in patients homozygous for the 460Trp allele compared with patients with the Gly460Gly genotype on low sodium diet but no differences were found at the higher sodium intake .
	manualset3
266982	5	426760	16	NULL	NULL	NULL	NULL	460Trp allele	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERPF , ERBF , and GFR were lower in patients homozygous for the 460Trp allele compared with patients with the Gly460Gly genotype on low sodium diet but no differences were found at the higher sodium intake .
	manualset3
266983	6	426760	16	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERPF , ERBF , and GFR were lower in patients homozygous for the 460Trp allele compared with patients with the Gly460Gly genotype on low sodium diet but no differences were found at the higher sodium intake .
	manualset3
266984	7	426760	16	NULL	NULL	NULL	NULL	Gly460Gly genotype	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERPF , ERBF , and GFR were lower in patients homozygous for the 460Trp allele compared with patients with the Gly460Gly genotype on low sodium diet but no differences were found at the higher sodium intake .
	manualset3
266985	8	426760	16	NULL	NULL	NULL	NULL	low sodium diet	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERPF , ERBF , and GFR were lower in patients homozygous for the 460Trp allele compared with patients with the Gly460Gly genotype on low sodium diet but no differences were found at the higher sodium intake .
	manualset3
266986	9	426760	16	NULL	NULL	NULL	NULL	differences	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERPF , ERBF , and GFR were lower in patients homozygous for the 460Trp allele compared with patients with the Gly460Gly genotype on low sodium diet but no differences were found at the higher sodium intake .
	manualset3
266987	10	426760	16	NULL	NULL	NULL	NULL	higher sodium intake	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ERPF , ERBF , and GFR were lower in patients homozygous for the 460Trp allele compared with patients with the Gly460Gly genotype on low sodium diet but no differences were found at the higher sodium intake .
	manualset3
266988	1	426761	16	NULL	NULL	NULL	NULL	differences	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Our differences of opinion ) .
	manualset3
266989	2	426761	16	NULL	NULL	NULL	NULL	opinion	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Our differences of opinion ) .
	manualset3
266990	1	426762	16	NULL	NULL	NULL	NULL	ES2	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ES2 was obtained in all but one ( control ) subject and the control ES2 duration mean was 33.5 ( SD 8.5 ) ms ( 80 % EMG amplitude reduction criterion ) .
	manualset3
266991	2	426762	16	NULL	NULL	NULL	NULL	one ( control ) subject	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ES2 was obtained in all but one ( control ) subject and the control ES2 duration mean was 33.5 ( SD 8.5 ) ms ( 80 % EMG amplitude reduction criterion ) .
	manualset3
266992	2	426762	16	NULL	NULL	NULL	NULL	one ( control ) subject	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ES2 was obtained in all but one ( control ) subject and the control ES2 duration mean was 33.5 ( SD 8.5 ) ms ( 80 % EMG amplitude reduction criterion ) .
	manualset3
266993	3	426762	16	NULL	NULL	NULL	NULL	control ES2 duration	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ES2 was obtained in all but one ( control ) subject and the control ES2 duration mean was 33.5 ( SD 8.5 ) ms ( 80 % EMG amplitude reduction criterion ) .
	manualset3
266994	4	426762	16	NULL	NULL	NULL	NULL	33.5 ( SD 8.5 ) ms	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ES2 was obtained in all but one ( control ) subject and the control ES2 duration mean was 33.5 ( SD 8.5 ) ms ( 80 % EMG amplitude reduction criterion ) .
	manualset3
266995	5	426762	16	NULL	NULL	NULL	NULL	80 % EMG amplitude reduction criterion	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ES2 was obtained in all but one ( control ) subject and the control ES2 duration mean was 33.5 ( SD 8.5 ) ms ( 80 % EMG amplitude reduction criterion ) .
	manualset3
266996	1	426763	16	NULL	NULL	NULL	NULL	ETA activation	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ETA activation mediates angiotensin II-induced infiltration of renal cortical T cells .
	manualset3
266997	2	426763	16	NULL	NULL	NULL	NULL	angiotensin II-induced infiltration	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ETA activation mediates angiotensin II-induced infiltration of renal cortical T cells .
	manualset3
266998	3	426763	16	NULL	NULL	NULL	NULL	renal cortical T cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	ETA activation mediates angiotensin II-induced infiltration of renal cortical T cells .
	manualset3
266999	1	426764	16	NULL	NULL	NULL	NULL	EUS-guided FNA	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EUS-guided FNA for the diagnosis of GI stromal cell tumors : sensitivity and cytologic yield .
	manualset3
267000	2	426764	16	NULL	NULL	NULL	NULL	diagnosis	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EUS-guided FNA for the diagnosis of GI stromal cell tumors : sensitivity and cytologic yield .
	manualset3
267001	3	426764	16	NULL	NULL	NULL	NULL	GI stromal cell tumors	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EUS-guided FNA for the diagnosis of GI stromal cell tumors : sensitivity and cytologic yield .
	manualset3
267002	4	426764	16	NULL	NULL	NULL	NULL	sensitivity	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EUS-guided FNA for the diagnosis of GI stromal cell tumors : sensitivity and cytologic yield .
	manualset3
267003	5	426764	16	NULL	NULL	NULL	NULL	cytologic yield	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EUS-guided FNA for the diagnosis of GI stromal cell tumors : sensitivity and cytologic yield .
	manualset3
267004	1	426765	16	NULL	NULL	NULL	NULL	EXPERIENCE	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EXPERIENCE TO DATE : The program is in use at more than 30 health care organization facilities and systems .
	manualset3
267005	2	426765	16	NULL	NULL	NULL	NULL	DATE	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EXPERIENCE TO DATE : The program is in use at more than 30 health care organization facilities and systems .
	manualset3
267006	3	426765	16	NULL	NULL	NULL	NULL	program	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EXPERIENCE TO DATE : The program is in use at more than 30 health care organization facilities and systems .
	manualset3
267007	4	426765	16	NULL	NULL	NULL	NULL	use	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EXPERIENCE TO DATE : The program is in use at more than 30 health care organization facilities and systems .
	manualset3
267008	5	426765	16	NULL	NULL	NULL	NULL	30	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EXPERIENCE TO DATE : The program is in use at more than 30 health care organization facilities and systems .
	manualset3
267009	6	426765	16	NULL	NULL	NULL	NULL	health care organization facilities	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EXPERIENCE TO DATE : The program is in use at more than 30 health care organization facilities and systems .
	manualset3
267010	7	426765	16	NULL	NULL	NULL	NULL	systems	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EXPERIENCE TO DATE : The program is in use at more than 30 health care organization facilities and systems .
	manualset3
267011	1	426766	16	NULL	NULL	NULL	NULL	EXPERIENCES	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EXPERIENCES : The server - based medical communication systems ( AFIP , iPATH , UICC-TPCC ) have been reported to be a useful and easy to handle tool for expert consultation .
	manualset3
267012	2	426766	16	NULL	NULL	NULL	NULL	server - based medical communication systems	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EXPERIENCES : The server - based medical communication systems ( AFIP , iPATH , UICC-TPCC ) have been reported to be a useful and easy to handle tool for expert consultation .
	manualset3
267013	3	426766	16	NULL	NULL	NULL	NULL	AFIP	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EXPERIENCES : The server - based medical communication systems ( AFIP , iPATH , UICC-TPCC ) have been reported to be a useful and easy to handle tool for expert consultation .
	manualset3
267014	4	426766	16	NULL	NULL	NULL	NULL	iPATH	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EXPERIENCES : The server - based medical communication systems ( AFIP , iPATH , UICC-TPCC ) have been reported to be a useful and easy to handle tool for expert consultation .
	manualset3
267015	5	426766	16	NULL	NULL	NULL	NULL	UICC-TPCC	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EXPERIENCES : The server - based medical communication systems ( AFIP , iPATH , UICC-TPCC ) have been reported to be a useful and easy to handle tool for expert consultation .
	manualset3
267016	6	426766	16	NULL	NULL	NULL	NULL	tool	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EXPERIENCES : The server - based medical communication systems ( AFIP , iPATH , UICC-TPCC ) have been reported to be a useful and easy to handle tool for expert consultation .
	manualset3
267017	7	426766	16	NULL	NULL	NULL	NULL	expert consultation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	EXPERIENCES : The server - based medical communication systems ( AFIP , iPATH , UICC-TPCC ) have been reported to be a useful and easy to handle tool for expert consultation .
	manualset3
267018	1	426767	16	NULL	NULL	NULL	NULL	ACT raw material lot	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each ACT raw material lot , however , also contained two predominant species : 55 , 106 + / - 111 and 51 , 414 + / - 32 Da .
	manualset3
267019	2	426767	16	NULL	NULL	NULL	NULL	two predominant species	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each ACT raw material lot , however , also contained two predominant species : 55 , 106 + / - 111 and 51 , 414 + / - 32 Da .
	manualset3
267020	3	426767	16	NULL	NULL	NULL	NULL	55 , 106 + / - 111 Da	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each ACT raw material lot , however , also contained two predominant species : 55 , 106 + / - 111 and 51 , 414 + / - 32 Da .
	manualset3
267021	4	426767	16	NULL	NULL	NULL	NULL	51 , 414 + / - 32 Da	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each ACT raw material lot , however , also contained two predominant species : 55 , 106 + / - 111 and 51 , 414 + / - 32 Da .
	manualset3
267022	1	426768	16	NULL	NULL	NULL	NULL	LN	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each LN was serially sectioned , and every set of three serial sections were tested for routine histopathological ( H & E ) and immunohistochemical examination with anti-cytokeratin antibodies ( IHC ) , and RT-LAMP analysis targeted cytokeratin 19 mRNA .
	manualset3
267023	2	426768	16	NULL	NULL	NULL	NULL	set	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each LN was serially sectioned , and every set of three serial sections were tested for routine histopathological ( H & E ) and immunohistochemical examination with anti-cytokeratin antibodies ( IHC ) , and RT-LAMP analysis targeted cytokeratin 19 mRNA .
	manualset3
267024	3	426768	16	NULL	NULL	NULL	NULL	three serial sections	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each LN was serially sectioned , and every set of three serial sections were tested for routine histopathological ( H & E ) and immunohistochemical examination with anti-cytokeratin antibodies ( IHC ) , and RT-LAMP analysis targeted cytokeratin 19 mRNA .
	manualset3
267025	4	426768	16	NULL	NULL	NULL	NULL	histopathological ( H & E ) and immunohistochemical examination	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each LN was serially sectioned , and every set of three serial sections were tested for routine histopathological ( H & E ) and immunohistochemical examination with anti-cytokeratin antibodies ( IHC ) , and RT-LAMP analysis targeted cytokeratin 19 mRNA .
	manualset3
267026	5	426768	16	NULL	NULL	NULL	NULL	anti-cytokeratin antibodies	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each LN was serially sectioned , and every set of three serial sections were tested for routine histopathological ( H & E ) and immunohistochemical examination with anti-cytokeratin antibodies ( IHC ) , and RT-LAMP analysis targeted cytokeratin 19 mRNA .
	manualset3
267027	6	426768	16	NULL	NULL	NULL	NULL	IHC	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each LN was serially sectioned , and every set of three serial sections were tested for routine histopathological ( H & E ) and immunohistochemical examination with anti-cytokeratin antibodies ( IHC ) , and RT-LAMP analysis targeted cytokeratin 19 mRNA .
	manualset3
267028	7	426768	16	NULL	NULL	NULL	NULL	RT-LAMP analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each LN was serially sectioned , and every set of three serial sections were tested for routine histopathological ( H & E ) and immunohistochemical examination with anti-cytokeratin antibodies ( IHC ) , and RT-LAMP analysis targeted cytokeratin 19 mRNA .
	manualset3
267029	8	426768	16	NULL	NULL	NULL	NULL	cytokeratin 19 mRNA	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each LN was serially sectioned , and every set of three serial sections were tested for routine histopathological ( H & E ) and immunohistochemical examination with anti-cytokeratin antibodies ( IHC ) , and RT-LAMP analysis targeted cytokeratin 19 mRNA .
	manualset3
267030	1	426769	16	NULL	NULL	NULL	NULL	compound	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each compound was tested for its effect on metabolic cooperation and also for its ability to reverse or modify the inhibitory properties of PMA on intercellular communication at noncytotoxic exposure concentrations .
	manualset3
267031	2	426769	16	NULL	NULL	NULL	NULL	effect	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each compound was tested for its effect on metabolic cooperation and also for its ability to reverse or modify the inhibitory properties of PMA on intercellular communication at noncytotoxic exposure concentrations .
	manualset3
267032	3	426769	16	NULL	NULL	NULL	NULL	metabolic cooperation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each compound was tested for its effect on metabolic cooperation and also for its ability to reverse or modify the inhibitory properties of PMA on intercellular communication at noncytotoxic exposure concentrations .
	manualset3
267033	4	426769	16	NULL	NULL	NULL	NULL	ability	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each compound was tested for its effect on metabolic cooperation and also for its ability to reverse or modify the inhibitory properties of PMA on intercellular communication at noncytotoxic exposure concentrations .
	manualset3
267034	5	426769	16	NULL	NULL	NULL	NULL	inhibitory properties	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each compound was tested for its effect on metabolic cooperation and also for its ability to reverse or modify the inhibitory properties of PMA on intercellular communication at noncytotoxic exposure concentrations .
	manualset3
267035	6	426769	16	NULL	NULL	NULL	NULL	PMA	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each compound was tested for its effect on metabolic cooperation and also for its ability to reverse or modify the inhibitory properties of PMA on intercellular communication at noncytotoxic exposure concentrations .
	manualset3
267036	7	426769	16	NULL	NULL	NULL	NULL	intercellular communication	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each compound was tested for its effect on metabolic cooperation and also for its ability to reverse or modify the inhibitory properties of PMA on intercellular communication at noncytotoxic exposure concentrations .
	manualset3
267037	8	426769	16	NULL	NULL	NULL	NULL	noncytotoxic exposure concentrations	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each compound was tested for its effect on metabolic cooperation and also for its ability to reverse or modify the inhibitory properties of PMA on intercellular communication at noncytotoxic exposure concentrations .
	manualset3
267038	1	426770	16	NULL	NULL	NULL	NULL	experience	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Our experience with choledochoduodenostomy ) .
	manualset3
267039	2	426770	16	NULL	NULL	NULL	NULL	choledochoduodenostomy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Our experience with choledochoduodenostomy ) .
	manualset3
267040	1	426771	16	NULL	NULL	NULL	NULL	form	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each form contains 1 mol of FMN/mol of apoprotein , exhibits a typical flavodoxin u.v.-visible absorption spectrum and does not contain covalently bound phosphate .
	manualset3
267041	2	426771	16	NULL	NULL	NULL	NULL	1 mol of FMN/mol of apoprotein	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each form contains 1 mol of FMN/mol of apoprotein , exhibits a typical flavodoxin u.v.-visible absorption spectrum and does not contain covalently bound phosphate .
	manualset3
267042	3	426771	16	NULL	NULL	NULL	NULL	flavodoxin u.v.-visible absorption spectrum	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each form contains 1 mol of FMN/mol of apoprotein , exhibits a typical flavodoxin u.v.-visible absorption spectrum and does not contain covalently bound phosphate .
	manualset3
267043	4	426771	16	NULL	NULL	NULL	NULL	covalently bound phosphate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each form contains 1 mol of FMN/mol of apoprotein , exhibits a typical flavodoxin u.v.-visible absorption spectrum and does not contain covalently bound phosphate .
	manualset3
267044	1	426772	16	NULL	NULL	NULL	NULL	hly determinant	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each hly determinant is independently deleted at a frequency of 10 ( -4 ) , leading to variants which exhibit similar levels of internal hemolysin but different amounts of secreted hemolysin .
	manualset3
267045	2	426772	16	NULL	NULL	NULL	NULL	frequency	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each hly determinant is independently deleted at a frequency of 10 ( -4 ) , leading to variants which exhibit similar levels of internal hemolysin but different amounts of secreted hemolysin .
	manualset3
267046	3	426772	16	NULL	NULL	NULL	NULL	10 ( -4 )	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each hly determinant is independently deleted at a frequency of 10 ( -4 ) , leading to variants which exhibit similar levels of internal hemolysin but different amounts of secreted hemolysin .
	manualset3
267047	4	426772	16	NULL	NULL	NULL	NULL	variants	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each hly determinant is independently deleted at a frequency of 10 ( -4 ) , leading to variants which exhibit similar levels of internal hemolysin but different amounts of secreted hemolysin .
	manualset3
267048	5	426772	16	NULL	NULL	NULL	NULL	levels	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each hly determinant is independently deleted at a frequency of 10 ( -4 ) , leading to variants which exhibit similar levels of internal hemolysin but different amounts of secreted hemolysin .
	manualset3
267049	6	426772	16	NULL	NULL	NULL	NULL	internal hemolysin	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each hly determinant is independently deleted at a frequency of 10 ( -4 ) , leading to variants which exhibit similar levels of internal hemolysin but different amounts of secreted hemolysin .
	manualset3
267050	7	426772	16	NULL	NULL	NULL	NULL	amounts	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each hly determinant is independently deleted at a frequency of 10 ( -4 ) , leading to variants which exhibit similar levels of internal hemolysin but different amounts of secreted hemolysin .
	manualset3
267051	8	426772	16	NULL	NULL	NULL	NULL	secreted hemolysin	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each hly determinant is independently deleted at a frequency of 10 ( -4 ) , leading to variants which exhibit similar levels of internal hemolysin but different amounts of secreted hemolysin .
	manualset3
267052	1	426773	16	NULL	NULL	NULL	NULL	wild-type levels	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each is necessary , but neither is sufficient for wild-type levels of his3 expression .
	manualset3
267053	2	426773	16	NULL	NULL	NULL	NULL	his3 expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each is necessary , but neither is sufficient for wild-type levels of his3 expression .
	manualset3
267054	1	426774	16	NULL	NULL	NULL	NULL	locus	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each locus was polymorphic , with the number of alleles ranging from two to 16 in C. sonorensis and from four to 18 in C. insularis .
	manualset3
267055	2	426774	16	NULL	NULL	NULL	NULL	number	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each locus was polymorphic , with the number of alleles ranging from two to 16 in C. sonorensis and from four to 18 in C. insularis .
	manualset3
267056	3	426774	16	NULL	NULL	NULL	NULL	alleles	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each locus was polymorphic , with the number of alleles ranging from two to 16 in C. sonorensis and from four to 18 in C. insularis .
	manualset3
267057	4	426774	16	NULL	NULL	NULL	NULL	two to 16	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each locus was polymorphic , with the number of alleles ranging from two to 16 in C. sonorensis and from four to 18 in C. insularis .
	manualset3
267058	5	426774	16	NULL	NULL	NULL	NULL	C. sonorensis	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each locus was polymorphic , with the number of alleles ranging from two to 16 in C. sonorensis and from four to 18 in C. insularis .
	manualset3
267059	6	426774	16	NULL	NULL	NULL	NULL	four to 18	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each locus was polymorphic , with the number of alleles ranging from two to 16 in C. sonorensis and from four to 18 in C. insularis .
	manualset3
267060	7	426774	16	NULL	NULL	NULL	NULL	C. insularis	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each locus was polymorphic , with the number of alleles ranging from two to 16 in C. sonorensis and from four to 18 in C. insularis .
	manualset3
267061	1	426775	16	NULL	NULL	NULL	NULL	histidine mutants	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each of the histidine mutants of Saccharomyces cerevisiae has been correlated with a particular step in histidine biosynthesis .
	manualset3
267062	2	426775	16	NULL	NULL	NULL	NULL	Saccharomyces cerevisiae	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each of the histidine mutants of Saccharomyces cerevisiae has been correlated with a particular step in histidine biosynthesis .
	manualset3
267063	3	426775	16	NULL	NULL	NULL	NULL	particular step	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each of the histidine mutants of Saccharomyces cerevisiae has been correlated with a particular step in histidine biosynthesis .
	manualset3
267064	4	426775	16	NULL	NULL	NULL	NULL	histidine biosynthesis	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each of the histidine mutants of Saccharomyces cerevisiae has been correlated with a particular step in histidine biosynthesis .
	manualset3
267065	1	426776	16	NULL	NULL	NULL	NULL	analogs	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each of these analogs was screened in the P388 lymphocytic leukemia system at the same time as indicine N-oxide , and the results were compared .
	manualset3
267066	2	426776	16	NULL	NULL	NULL	NULL	P388 lymphocytic leukemia system	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each of these analogs was screened in the P388 lymphocytic leukemia system at the same time as indicine N-oxide , and the results were compared .
	manualset3
267067	3	426776	16	NULL	NULL	NULL	NULL	indicine N-oxide	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each of these analogs was screened in the P388 lymphocytic leukemia system at the same time as indicine N-oxide , and the results were compared .
	manualset3
267068	4	426776	16	NULL	NULL	NULL	NULL	results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each of these analogs was screened in the P388 lymphocytic leukemia system at the same time as indicine N-oxide , and the results were compared .
	manualset3
267071	1	426779	16	NULL	NULL	NULL	NULL	subject	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each subject was clamped at both the `` normal '' and `` obese '' OGTT insulin profiles .
	manualset3
267072	2	426779	16	NULL	NULL	NULL	NULL	`` normal '' OGTT insulin profiles	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each subject was clamped at both the `` normal '' and `` obese '' OGTT insulin profiles .
	manualset3
267073	3	426779	16	NULL	NULL	NULL	NULL	`` obese '' OGTT insulin profiles	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Each subject was clamped at both the `` normal '' and `` obese '' OGTT insulin profiles .
	manualset3
267074	1	426780	16	NULL	NULL	NULL	NULL	first time	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier for the first time we identified the adhesion molecules with physico-chemical and biological properties much different from other known cell adhesion molecules of bovine eye .
	manualset3
267075	2	426780	16	NULL	NULL	NULL	NULL	adhesion molecules	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier for the first time we identified the adhesion molecules with physico-chemical and biological properties much different from other known cell adhesion molecules of bovine eye .
	manualset3
267076	3	426780	16	NULL	NULL	NULL	NULL	physico-chemical properties	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier for the first time we identified the adhesion molecules with physico-chemical and biological properties much different from other known cell adhesion molecules of bovine eye .
	manualset3
267077	4	426780	16	NULL	NULL	NULL	NULL	biological properties	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier for the first time we identified the adhesion molecules with physico-chemical and biological properties much different from other known cell adhesion molecules of bovine eye .
	manualset3
267078	5	426780	16	NULL	NULL	NULL	NULL	cell adhesion molecules	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier for the first time we identified the adhesion molecules with physico-chemical and biological properties much different from other known cell adhesion molecules of bovine eye .
	manualset3
267079	6	426780	16	NULL	NULL	NULL	NULL	bovine eye	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier for the first time we identified the adhesion molecules with physico-chemical and biological properties much different from other known cell adhesion molecules of bovine eye .
	manualset3
267080	1	426781	16	NULL	NULL	NULL	NULL	response assessment	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier response assessment in invasive aspergillosis based on the kinetics of serum Aspergillus galactomannan : proposal for a new definition .
	manualset3
267081	2	426781	16	NULL	NULL	NULL	NULL	invasive aspergillosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier response assessment in invasive aspergillosis based on the kinetics of serum Aspergillus galactomannan : proposal for a new definition .
	manualset3
267082	3	426781	16	NULL	NULL	NULL	NULL	kinetics	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier response assessment in invasive aspergillosis based on the kinetics of serum Aspergillus galactomannan : proposal for a new definition .
	manualset3
267083	4	426781	16	NULL	NULL	NULL	NULL	serum Aspergillus galactomannan	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier response assessment in invasive aspergillosis based on the kinetics of serum Aspergillus galactomannan : proposal for a new definition .
	manualset3
267084	5	426781	16	NULL	NULL	NULL	NULL	proposal	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier response assessment in invasive aspergillosis based on the kinetics of serum Aspergillus galactomannan : proposal for a new definition .
	manualset3
267085	6	426781	16	NULL	NULL	NULL	NULL	definition	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier response assessment in invasive aspergillosis based on the kinetics of serum Aspergillus galactomannan : proposal for a new definition .
	manualset3
267086	1	426782	16	NULL	NULL	NULL	NULL	studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier studies in which X-linked gene activities were monitored in msl/msl male larvae demonstrated that these genes are responsible for setting and/or maintaining the level of X chromosome transcription in males ( i.e. , they are necessary for proper dosage compensation ) .
	manualset3
267087	2	426782	16	NULL	NULL	NULL	NULL	X-linked gene activities	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier studies in which X-linked gene activities were monitored in msl/msl male larvae demonstrated that these genes are responsible for setting and/or maintaining the level of X chromosome transcription in males ( i.e. , they are necessary for proper dosage compensation ) .
	manualset3
267088	3	426782	16	NULL	NULL	NULL	NULL	msl/msl male larvae	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier studies in which X-linked gene activities were monitored in msl/msl male larvae demonstrated that these genes are responsible for setting and/or maintaining the level of X chromosome transcription in males ( i.e. , they are necessary for proper dosage compensation ) .
	manualset3
267089	4	426782	16	NULL	NULL	NULL	NULL	genes	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier studies in which X-linked gene activities were monitored in msl/msl male larvae demonstrated that these genes are responsible for setting and/or maintaining the level of X chromosome transcription in males ( i.e. , they are necessary for proper dosage compensation ) .
	manualset3
267091	6	426782	16	NULL	NULL	NULL	NULL	level	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier studies in which X-linked gene activities were monitored in msl/msl male larvae demonstrated that these genes are responsible for setting and/or maintaining the level of X chromosome transcription in males ( i.e. , they are necessary for proper dosage compensation ) .
	manualset3
267092	7	426782	16	NULL	NULL	NULL	NULL	X chromosome transcription	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier studies in which X-linked gene activities were monitored in msl/msl male larvae demonstrated that these genes are responsible for setting and/or maintaining the level of X chromosome transcription in males ( i.e. , they are necessary for proper dosage compensation ) .
	manualset3
267093	8	426782	16	NULL	NULL	NULL	NULL	males	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier studies in which X-linked gene activities were monitored in msl/msl male larvae demonstrated that these genes are responsible for setting and/or maintaining the level of X chromosome transcription in males ( i.e. , they are necessary for proper dosage compensation ) .
	manualset3
267094	9	426782	16	NULL	NULL	NULL	NULL	dosage compensation	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier studies in which X-linked gene activities were monitored in msl/msl male larvae demonstrated that these genes are responsible for setting and/or maintaining the level of X chromosome transcription in males ( i.e. , they are necessary for proper dosage compensation ) .
	manualset3
267095	1	426783	16	NULL	NULL	NULL	NULL	studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier studies revealed normal karyotypes in peripheral blood cultures of male breast cancer patients and abnormalities only in the tumor tissue .
	manualset3
267096	2	426783	16	NULL	NULL	NULL	NULL	normal karyotypes	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier studies revealed normal karyotypes in peripheral blood cultures of male breast cancer patients and abnormalities only in the tumor tissue .
	manualset3
267097	3	426783	16	NULL	NULL	NULL	NULL	peripheral blood cultures	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier studies revealed normal karyotypes in peripheral blood cultures of male breast cancer patients and abnormalities only in the tumor tissue .
	manualset3
267098	4	426783	16	NULL	NULL	NULL	NULL	male breast cancer patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier studies revealed normal karyotypes in peripheral blood cultures of male breast cancer patients and abnormalities only in the tumor tissue .
	manualset3
267099	5	426783	16	NULL	NULL	NULL	NULL	abnormalities	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier studies revealed normal karyotypes in peripheral blood cultures of male breast cancer patients and abnormalities only in the tumor tissue .
	manualset3
267100	6	426783	16	NULL	NULL	NULL	NULL	tumor tissue	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier studies revealed normal karyotypes in peripheral blood cultures of male breast cancer patients and abnormalities only in the tumor tissue .
	manualset3
267101	1	426784	16	NULL	NULL	NULL	NULL	work	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier work demonstrated that in this system double strand break repair takes place via incorporation of a patch of DNA into a gap formed at the break site .
	manualset3
267102	2	426784	16	NULL	NULL	NULL	NULL	system	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier work demonstrated that in this system double strand break repair takes place via incorporation of a patch of DNA into a gap formed at the break site .
	manualset3
267103	3	426784	16	NULL	NULL	NULL	NULL	double strand break repair	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier work demonstrated that in this system double strand break repair takes place via incorporation of a patch of DNA into a gap formed at the break site .
	manualset3
267104	4	426784	16	NULL	NULL	NULL	NULL	incorporation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier work demonstrated that in this system double strand break repair takes place via incorporation of a patch of DNA into a gap formed at the break site .
	manualset3
267105	5	426784	16	NULL	NULL	NULL	NULL	patch of DNA	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier work demonstrated that in this system double strand break repair takes place via incorporation of a patch of DNA into a gap formed at the break site .
	manualset3
267106	6	426784	16	NULL	NULL	NULL	NULL	gap	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier work demonstrated that in this system double strand break repair takes place via incorporation of a patch of DNA into a gap formed at the break site .
	manualset3
267107	7	426784	16	NULL	NULL	NULL	NULL	break site	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier work demonstrated that in this system double strand break repair takes place via incorporation of a patch of DNA into a gap formed at the break site .
	manualset3
267108	1	426785	16	NULL	NULL	NULL	NULL	increase	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier , a similar increase in binding of antibody specific for pyrimidine ( 6-4 ) pyrimidone photoproducts to undenatured DNA isolated from UV-irradiated Chinese hamster ovary cells was reported ( Mitchell et al. , 1986 ) .
	manualset3
267109	2	426785	16	NULL	NULL	NULL	NULL	binding	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier , a similar increase in binding of antibody specific for pyrimidine ( 6-4 ) pyrimidone photoproducts to undenatured DNA isolated from UV-irradiated Chinese hamster ovary cells was reported ( Mitchell et al. , 1986 ) .
	manualset3
267110	3	426785	16	NULL	NULL	NULL	NULL	antibody specific	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier , a similar increase in binding of antibody specific for pyrimidine ( 6-4 ) pyrimidone photoproducts to undenatured DNA isolated from UV-irradiated Chinese hamster ovary cells was reported ( Mitchell et al. , 1986 ) .
	manualset3
267111	4	426785	16	NULL	NULL	NULL	NULL	pyrimidine ( 6-4 ) pyrimidone photoproducts	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier , a similar increase in binding of antibody specific for pyrimidine ( 6-4 ) pyrimidone photoproducts to undenatured DNA isolated from UV-irradiated Chinese hamster ovary cells was reported ( Mitchell et al. , 1986 ) .
	manualset3
267112	5	426785	16	NULL	NULL	NULL	NULL	UV-irradiated Chinese hamster ovary cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier , a similar increase in binding of antibody specific for pyrimidine ( 6-4 ) pyrimidone photoproducts to undenatured DNA isolated from UV-irradiated Chinese hamster ovary cells was reported ( Mitchell et al. , 1986 ) .
	manualset3
267113	6	426785	16	NULL	NULL	NULL	NULL	Mitchell et al. , 1986	Citation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier , a similar increase in binding of antibody specific for pyrimidine ( 6-4 ) pyrimidone photoproducts to undenatured DNA isolated from UV-irradiated Chinese hamster ovary cells was reported ( Mitchell et al. , 1986 ) .
	manualset3
267114	1	426786	16	NULL	NULL	NULL	NULL	development	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier , we reported the development of a coumarin-based prodrug system that could be used for the preparation of cyclic prodrugs of opioid peptides .
	manualset3
267115	2	426786	16	NULL	NULL	NULL	NULL	coumarin-based prodrug system	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier , we reported the development of a coumarin-based prodrug system that could be used for the preparation of cyclic prodrugs of opioid peptides .
	manualset3
267116	3	426786	16	NULL	NULL	NULL	NULL	preparation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier , we reported the development of a coumarin-based prodrug system that could be used for the preparation of cyclic prodrugs of opioid peptides .
	manualset3
267117	4	426786	16	NULL	NULL	NULL	NULL	cyclic prodrugs	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier , we reported the development of a coumarin-based prodrug system that could be used for the preparation of cyclic prodrugs of opioid peptides .
	manualset3
267118	5	426786	16	NULL	NULL	NULL	NULL	opioid peptides	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Earlier , we reported the development of a coumarin-based prodrug system that could be used for the preparation of cyclic prodrugs of opioid peptides .
	manualset3
267119	1	426787	16	NULL	NULL	NULL	NULL	Early passage cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early passage cells contained Rb which was primarily hyperphosphorylated while cells in M0 contained Rb protein which was predominantly underphosphorylated .
	manualset3
267120	2	426787	16	NULL	NULL	NULL	NULL	Rb	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early passage cells contained Rb which was primarily hyperphosphorylated while cells in M0 contained Rb protein which was predominantly underphosphorylated .
	manualset3
267121	3	426787	16	NULL	NULL	NULL	NULL	cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early passage cells contained Rb which was primarily hyperphosphorylated while cells in M0 contained Rb protein which was predominantly underphosphorylated .
	manualset3
267122	4	426787	16	NULL	NULL	NULL	NULL	M0	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early passage cells contained Rb which was primarily hyperphosphorylated while cells in M0 contained Rb protein which was predominantly underphosphorylated .
	manualset3
267123	5	426787	16	NULL	NULL	NULL	NULL	Rb protein	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early passage cells contained Rb which was primarily hyperphosphorylated while cells in M0 contained Rb protein which was predominantly underphosphorylated .
	manualset3
267124	1	426788	16	NULL	NULL	NULL	NULL	Early detection	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early detection of abnormalities in the clot quality test and/or evidence of systemic bleeding followed by immediate correction of the clotting defects using specific antivenom can reduce morbidity in Russell 's viper envenomation .
	manualset3
267125	2	426788	16	NULL	NULL	NULL	NULL	abnormalities	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early detection of abnormalities in the clot quality test and/or evidence of systemic bleeding followed by immediate correction of the clotting defects using specific antivenom can reduce morbidity in Russell 's viper envenomation .
	manualset3
267126	3	426788	16	NULL	NULL	NULL	NULL	clot quality test	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early detection of abnormalities in the clot quality test and/or evidence of systemic bleeding followed by immediate correction of the clotting defects using specific antivenom can reduce morbidity in Russell 's viper envenomation .
	manualset3
267127	4	426788	16	NULL	NULL	NULL	NULL	evidence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early detection of abnormalities in the clot quality test and/or evidence of systemic bleeding followed by immediate correction of the clotting defects using specific antivenom can reduce morbidity in Russell 's viper envenomation .
	manualset3
267128	5	426788	16	NULL	NULL	NULL	NULL	systemic bleeding	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early detection of abnormalities in the clot quality test and/or evidence of systemic bleeding followed by immediate correction of the clotting defects using specific antivenom can reduce morbidity in Russell 's viper envenomation .
	manualset3
267129	6	426788	16	NULL	NULL	NULL	NULL	immediate correction	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early detection of abnormalities in the clot quality test and/or evidence of systemic bleeding followed by immediate correction of the clotting defects using specific antivenom can reduce morbidity in Russell 's viper envenomation .
	manualset3
267130	7	426788	16	NULL	NULL	NULL	NULL	clotting defects	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early detection of abnormalities in the clot quality test and/or evidence of systemic bleeding followed by immediate correction of the clotting defects using specific antivenom can reduce morbidity in Russell 's viper envenomation .
	manualset3
267131	8	426788	16	NULL	NULL	NULL	NULL	specific antivenom	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early detection of abnormalities in the clot quality test and/or evidence of systemic bleeding followed by immediate correction of the clotting defects using specific antivenom can reduce morbidity in Russell 's viper envenomation .
	manualset3
267132	9	426788	16	NULL	NULL	NULL	NULL	morbidity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early detection of abnormalities in the clot quality test and/or evidence of systemic bleeding followed by immediate correction of the clotting defects using specific antivenom can reduce morbidity in Russell 's viper envenomation .
	manualset3
267133	10	426788	16	NULL	NULL	NULL	NULL	Russell 's viper	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early detection of abnormalities in the clot quality test and/or evidence of systemic bleeding followed by immediate correction of the clotting defects using specific antivenom can reduce morbidity in Russell 's viper envenomation .
	manualset3
267134	11	426788	16	NULL	NULL	NULL	NULL	envenomation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early detection of abnormalities in the clot quality test and/or evidence of systemic bleeding followed by immediate correction of the clotting defects using specific antivenom can reduce morbidity in Russell 's viper envenomation .
	manualset3
267135	1	426789	16	NULL	NULL	NULL	NULL	development	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early development of beta-cells is impaired in the GK rat model of type 2 diabetes .
	manualset3
267136	2	426789	16	NULL	NULL	NULL	NULL	beta-cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early development of beta-cells is impaired in the GK rat model of type 2 diabetes .
	manualset3
267137	3	426789	16	NULL	NULL	NULL	NULL	GK rat model	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early development of beta-cells is impaired in the GK rat model of type 2 diabetes .
	manualset3
267138	4	426789	16	NULL	NULL	NULL	NULL	type 2 diabetes	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early development of beta-cells is impaired in the GK rat model of type 2 diabetes .
	manualset3
267139	1	426790	16	NULL	NULL	NULL	NULL	Early development	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early development of injection-site sarcomas in rats : a study of tumors induced by iron-dextran .
	manualset3
267140	2	426790	16	NULL	NULL	NULL	NULL	injection-site sarcomas	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early development of injection-site sarcomas in rats : a study of tumors induced by iron-dextran .
	manualset3
267141	3	426790	16	NULL	NULL	NULL	NULL	rats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early development of injection-site sarcomas in rats : a study of tumors induced by iron-dextran .
	manualset3
267142	4	426790	16	NULL	NULL	NULL	NULL	study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early development of injection-site sarcomas in rats : a study of tumors induced by iron-dextran .
	manualset3
267143	5	426790	16	NULL	NULL	NULL	NULL	tumors	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early development of injection-site sarcomas in rats : a study of tumors induced by iron-dextran .
	manualset3
267144	6	426790	16	NULL	NULL	NULL	NULL	iron-dextran	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early development of injection-site sarcomas in rats : a study of tumors induced by iron-dextran .
	manualset3
267145	1	426791	16	NULL	NULL	NULL	NULL	Oxygen saturation	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Oxygen saturation of arterial blood following pneumonectomy ) .
	manualset3
267146	2	426791	16	NULL	NULL	NULL	NULL	arterial blood	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Oxygen saturation of arterial blood following pneumonectomy ) .
	manualset3
267147	3	426791	16	NULL	NULL	NULL	NULL	pneumonectomy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Oxygen saturation of arterial blood following pneumonectomy ) .
	manualset3
267148	1	426792	16	NULL	NULL	NULL	NULL	Early effects	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early effects of 150-MEV proton irradiation in rhesus monkeys .
	manualset3
267149	2	426792	16	NULL	NULL	NULL	NULL	150-MEV	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early effects of 150-MEV proton irradiation in rhesus monkeys .
	manualset3
267150	3	426792	16	NULL	NULL	NULL	NULL	proton irradiation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early effects of 150-MEV proton irradiation in rhesus monkeys .
	manualset3
267151	4	426792	16	NULL	NULL	NULL	NULL	rhesus monkeys	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early effects of 150-MEV proton irradiation in rhesus monkeys .
	manualset3
267152	1	426793	16	NULL	NULL	NULL	NULL	indicators	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early indicators suggest increasing further the participation of union and non-union staff in decision-making on multiple levels , but with clearly defined `` boundaries of responsibility . ''
	manualset3
267153	2	426793	16	NULL	NULL	NULL	NULL	participation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early indicators suggest increasing further the participation of union and non-union staff in decision-making on multiple levels , but with clearly defined `` boundaries of responsibility . ''
	manualset3
267154	3	426793	16	NULL	NULL	NULL	NULL	union staff	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early indicators suggest increasing further the participation of union and non-union staff in decision-making on multiple levels , but with clearly defined `` boundaries of responsibility . ''
	manualset3
267155	4	426793	16	NULL	NULL	NULL	NULL	non-union staff	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early indicators suggest increasing further the participation of union and non-union staff in decision-making on multiple levels , but with clearly defined `` boundaries of responsibility . ''
	manualset3
267156	5	426793	16	NULL	NULL	NULL	NULL	decision-making	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early indicators suggest increasing further the participation of union and non-union staff in decision-making on multiple levels , but with clearly defined `` boundaries of responsibility . ''
	manualset3
267157	6	426793	16	NULL	NULL	NULL	NULL	multiple levels	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early indicators suggest increasing further the participation of union and non-union staff in decision-making on multiple levels , but with clearly defined `` boundaries of responsibility . ''
	manualset3
267158	7	426793	16	NULL	NULL	NULL	NULL	boundaries of responsibility	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early indicators suggest increasing further the participation of union and non-union staff in decision-making on multiple levels , but with clearly defined `` boundaries of responsibility . ''
	manualset3
267159	1	426794	16	NULL	NULL	NULL	NULL	Early recognition	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early recognition of concurrent Lyme disease and HGE is important because amoxicillin , an antibiotic of choice for young children with early Lyme disease , is ineffective for HGE .
	manualset3
267160	2	426794	16	NULL	NULL	NULL	NULL	Lyme disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early recognition of concurrent Lyme disease and HGE is important because amoxicillin , an antibiotic of choice for young children with early Lyme disease , is ineffective for HGE .
	manualset3
267161	3	426794	16	NULL	NULL	NULL	NULL	HGE	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early recognition of concurrent Lyme disease and HGE is important because amoxicillin , an antibiotic of choice for young children with early Lyme disease , is ineffective for HGE .
	manualset3
267162	4	426794	16	NULL	NULL	NULL	NULL	amoxicillin	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early recognition of concurrent Lyme disease and HGE is important because amoxicillin , an antibiotic of choice for young children with early Lyme disease , is ineffective for HGE .
	manualset3
267163	5	426794	16	NULL	NULL	NULL	NULL	antibiotic	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early recognition of concurrent Lyme disease and HGE is important because amoxicillin , an antibiotic of choice for young children with early Lyme disease , is ineffective for HGE .
	manualset3
267164	6	426794	16	NULL	NULL	NULL	NULL	choice	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early recognition of concurrent Lyme disease and HGE is important because amoxicillin , an antibiotic of choice for young children with early Lyme disease , is ineffective for HGE .
	manualset3
267165	7	426794	16	NULL	NULL	NULL	NULL	young children	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early recognition of concurrent Lyme disease and HGE is important because amoxicillin , an antibiotic of choice for young children with early Lyme disease , is ineffective for HGE .
	manualset3
267166	8	426794	16	NULL	NULL	NULL	NULL	early Lyme disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early recognition of concurrent Lyme disease and HGE is important because amoxicillin , an antibiotic of choice for young children with early Lyme disease , is ineffective for HGE .
	manualset3
267167	9	426794	16	NULL	NULL	NULL	NULL	HGE	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early recognition of concurrent Lyme disease and HGE is important because amoxicillin , an antibiotic of choice for young children with early Lyme disease , is ineffective for HGE .
	manualset3
267168	1	426795	16	NULL	NULL	NULL	NULL	Early mobilisation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early mobilisation , aggressive chest physiotherapy and adequate pain control are essential components of effective postoperative care .
	manualset3
267169	2	426795	16	NULL	NULL	NULL	NULL	chest physiotherapy	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early mobilisation , aggressive chest physiotherapy and adequate pain control are essential components of effective postoperative care .
	manualset3
267170	3	426795	16	NULL	NULL	NULL	NULL	pain control	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early mobilisation , aggressive chest physiotherapy and adequate pain control are essential components of effective postoperative care .
	manualset3
267171	4	426795	16	NULL	NULL	NULL	NULL	essential components	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early mobilisation , aggressive chest physiotherapy and adequate pain control are essential components of effective postoperative care .
	manualset3
267172	5	426795	16	NULL	NULL	NULL	NULL	effective postoperative care	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early mobilisation , aggressive chest physiotherapy and adequate pain control are essential components of effective postoperative care .
	manualset3
267173	1	426796	16	NULL	NULL	NULL	NULL	Early results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early and late results of coronary artery bypass in patients with hyperlipoproteinemia .
	manualset3
267174	2	426796	16	NULL	NULL	NULL	NULL	late results	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early and late results of coronary artery bypass in patients with hyperlipoproteinemia .
	manualset3
267175	3	426796	16	NULL	NULL	NULL	NULL	coronary artery bypass	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early and late results of coronary artery bypass in patients with hyperlipoproteinemia .
	manualset3
267176	4	426796	16	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early and late results of coronary artery bypass in patients with hyperlipoproteinemia .
	manualset3
267177	5	426796	16	NULL	NULL	NULL	NULL	hyperlipoproteinemia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early and late results of coronary artery bypass in patients with hyperlipoproteinemia .
	manualset3
267178	1	426797	16	NULL	NULL	NULL	NULL	Early postoperative complications	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early postoperative complications amounted to 3.4 % .
	manualset3
267179	2	426797	16	NULL	NULL	NULL	NULL	3.4 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early postoperative complications amounted to 3.4 % .
	manualset3
267180	1	426798	16	NULL	NULL	NULL	NULL	Early hilar lung cancer	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early hilar lung cancer is rare .
	manualset3
267181	1	426799	16	NULL	NULL	NULL	NULL	Early operative morbidity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early operative morbidity and mortality in 1051 consecutive kidney transplants over 20 years at our centers .
	manualset3
267182	2	426799	16	NULL	NULL	NULL	NULL	Early operative mortality	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early operative morbidity and mortality in 1051 consecutive kidney transplants over 20 years at our centers .
	manualset3
267183	3	426799	16	NULL	NULL	NULL	NULL	1051	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early operative morbidity and mortality in 1051 consecutive kidney transplants over 20 years at our centers .
	manualset3
267184	4	426799	16	NULL	NULL	NULL	NULL	kidney transplants	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early operative morbidity and mortality in 1051 consecutive kidney transplants over 20 years at our centers .
	manualset3
267185	5	426799	16	NULL	NULL	NULL	NULL	20 years	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early operative morbidity and mortality in 1051 consecutive kidney transplants over 20 years at our centers .
	manualset3
267186	6	426799	16	NULL	NULL	NULL	NULL	centers	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early operative morbidity and mortality in 1051 consecutive kidney transplants over 20 years at our centers .
	manualset3
267187	1	426800	16	NULL	NULL	NULL	NULL	evaluation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early adequate evaluation of motor development and prognosis of degree of long-term motor disability is very important not only for parents , but also for correct management of goal oriented rehabilitation treatment and for planning of preventive measures .
	manualset3
267188	2	426800	16	NULL	NULL	NULL	NULL	motor development	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early adequate evaluation of motor development and prognosis of degree of long-term motor disability is very important not only for parents , but also for correct management of goal oriented rehabilitation treatment and for planning of preventive measures .
	manualset3
267189	3	426800	16	NULL	NULL	NULL	NULL	prognosis	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early adequate evaluation of motor development and prognosis of degree of long-term motor disability is very important not only for parents , but also for correct management of goal oriented rehabilitation treatment and for planning of preventive measures .
	manualset3
267190	4	426800	16	NULL	NULL	NULL	NULL	degree	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early adequate evaluation of motor development and prognosis of degree of long-term motor disability is very important not only for parents , but also for correct management of goal oriented rehabilitation treatment and for planning of preventive measures .
	manualset3
267191	5	426800	16	NULL	NULL	NULL	NULL	long-term motor disability	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early adequate evaluation of motor development and prognosis of degree of long-term motor disability is very important not only for parents , but also for correct management of goal oriented rehabilitation treatment and for planning of preventive measures .
	manualset3
267192	6	426800	16	NULL	NULL	NULL	NULL	parents	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early adequate evaluation of motor development and prognosis of degree of long-term motor disability is very important not only for parents , but also for correct management of goal oriented rehabilitation treatment and for planning of preventive measures .
	manualset3
267193	7	426800	16	NULL	NULL	NULL	NULL	correct management	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early adequate evaluation of motor development and prognosis of degree of long-term motor disability is very important not only for parents , but also for correct management of goal oriented rehabilitation treatment and for planning of preventive measures .
	manualset3
267194	8	426800	16	NULL	NULL	NULL	NULL	goal oriented rehabilitation treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early adequate evaluation of motor development and prognosis of degree of long-term motor disability is very important not only for parents , but also for correct management of goal oriented rehabilitation treatment and for planning of preventive measures .
	manualset3
267195	9	426800	16	NULL	NULL	NULL	NULL	planning	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early adequate evaluation of motor development and prognosis of degree of long-term motor disability is very important not only for parents , but also for correct management of goal oriented rehabilitation treatment and for planning of preventive measures .
	manualset3
267196	10	426800	16	NULL	NULL	NULL	NULL	preventive measures	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early adequate evaluation of motor development and prognosis of degree of long-term motor disability is very important not only for parents , but also for correct management of goal oriented rehabilitation treatment and for planning of preventive measures .
	manualset3
267210	1	426801	16	NULL	NULL	NULL	NULL	embryonic vascular patterning	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early embryonic vascular patterning by matrix-mediated paracrine signalling : a mathematical model study .
	manualset3
267211	2	426801	16	NULL	NULL	NULL	NULL	matrix-mediated paracrine signalling	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early embryonic vascular patterning by matrix-mediated paracrine signalling : a mathematical model study .
	manualset3
267212	3	426801	16	NULL	NULL	NULL	NULL	mathematical model study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early embryonic vascular patterning by matrix-mediated paracrine signalling : a mathematical model study .
	manualset3
267197	1	426802	16	NULL	NULL	NULL	NULL	maternal undernutrition	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early maternal undernutrition impaired secretion of insulin but maintained normal blood glucose levels until adulthood .
	manualset3
267198	2	426802	16	NULL	NULL	NULL	NULL	secretion	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early maternal undernutrition impaired secretion of insulin but maintained normal blood glucose levels until adulthood .
	manualset3
267199	3	426802	16	NULL	NULL	NULL	NULL	insulin	AminoAcidPeptide												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early maternal undernutrition impaired secretion of insulin but maintained normal blood glucose levels until adulthood .
	manualset3
267200	4	426802	16	NULL	NULL	NULL	NULL	normal blood glucose levels	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early maternal undernutrition impaired secretion of insulin but maintained normal blood glucose levels until adulthood .
	manualset3
267201	5	426802	16	NULL	NULL	NULL	NULL	adulthood	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early maternal undernutrition impaired secretion of insulin but maintained normal blood glucose levels until adulthood .
	manualset3
267202	1	426803	16	NULL	NULL	NULL	NULL	Early peritoneal mesothelioma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early peritoneal mesothelioma : a treatable malignancy .
	manualset3
267203	2	426803	16	NULL	NULL	NULL	NULL	treatable malignancy	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early peritoneal mesothelioma : a treatable malignancy .
	manualset3
267204	1	426804	16	NULL	NULL	NULL	NULL	Early surgical intervention	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early surgical intervention is recommended because of the risk of rupture .
	manualset3
267205	2	426804	16	NULL	NULL	NULL	NULL	risk	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early surgical intervention is recommended because of the risk of rupture .
	manualset3
267206	3	426804	16	NULL	NULL	NULL	NULL	rupture	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early surgical intervention is recommended because of the risk of rupture .
	manualset3
267207	1	426805	16	NULL	NULL	NULL	NULL	transplant-related mortality	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early transplant-related mortality was 25 % .
	manualset3
267208	2	426805	16	NULL	NULL	NULL	NULL	25 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Early transplant-related mortality was 25 % .
	manualset3
267209	1	426806	16	NULL	NULL	NULL	NULL	Eating disorders	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Eating disorders : a transcultural perspective .
	manualset3
267213	2	426806	16	NULL	NULL	NULL	NULL	transcultural perspective	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Eating disorders : a transcultural perspective .
	manualset3
267214	1	426807	16	NULL	NULL	NULL	NULL	Pacemaker infection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Pacemaker infection developed one month after the surgery for prosthetic valve endocarditis ) .
	manualset3
267215	2	426807	16	NULL	NULL	NULL	NULL	one month	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Pacemaker infection developed one month after the surgery for prosthetic valve endocarditis ) .
	manualset3
267216	3	426807	16	NULL	NULL	NULL	NULL	surgery	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Pacemaker infection developed one month after the surgery for prosthetic valve endocarditis ) .
	manualset3
267217	4	426807	16	NULL	NULL	NULL	NULL	prosthetic valve endocarditis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Pacemaker infection developed one month after the surgery for prosthetic valve endocarditis ) .
	manualset3
267218	1	426808	16	NULL	NULL	NULL	NULL	Ecdysone inducible gene	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ecdysone inducible gene , E75 is a primary target of ecdysone receptor ( EcR ) , and is found to play a critical role in the molting process of arthropods .
	manualset3
267219	2	426808	16	NULL	NULL	NULL	NULL	E75	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ecdysone inducible gene , E75 is a primary target of ecdysone receptor ( EcR ) , and is found to play a critical role in the molting process of arthropods .
	manualset3
267220	3	426808	16	NULL	NULL	NULL	NULL	primary target	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ecdysone inducible gene , E75 is a primary target of ecdysone receptor ( EcR ) , and is found to play a critical role in the molting process of arthropods .
	manualset3
267221	4	426808	16	NULL	NULL	NULL	NULL	ecdysone receptor ( EcR )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ecdysone inducible gene , E75 is a primary target of ecdysone receptor ( EcR ) , and is found to play a critical role in the molting process of arthropods .
	manualset3
267222	5	426808	16	NULL	NULL	NULL	NULL	role	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ecdysone inducible gene , E75 is a primary target of ecdysone receptor ( EcR ) , and is found to play a critical role in the molting process of arthropods .
	manualset3
267223	6	426808	16	NULL	NULL	NULL	NULL	molting process	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ecdysone inducible gene , E75 is a primary target of ecdysone receptor ( EcR ) , and is found to play a critical role in the molting process of arthropods .
	manualset3
267224	7	426808	16	NULL	NULL	NULL	NULL	arthropods	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ecdysone inducible gene , E75 is a primary target of ecdysone receptor ( EcR ) , and is found to play a critical role in the molting process of arthropods .
	manualset3
267225	1	426809	16	NULL	NULL	NULL	NULL	Echocardiographic data	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Echocardiographic and hemodynamic data were measured in closed-chest dogs during graded cardiac tamponade ( pericardial pressure 5 , 10 , and 15 mm Hg ) before and after production of diffuse ischemic left ventricular dysfunction .
	manualset3
267226	2	426809	16	NULL	NULL	NULL	NULL	hemodynamic data	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Echocardiographic and hemodynamic data were measured in closed-chest dogs during graded cardiac tamponade ( pericardial pressure 5 , 10 , and 15 mm Hg ) before and after production of diffuse ischemic left ventricular dysfunction .
	manualset3
267227	3	426809	16	NULL	NULL	NULL	NULL	closed-chest dogs	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Echocardiographic and hemodynamic data were measured in closed-chest dogs during graded cardiac tamponade ( pericardial pressure 5 , 10 , and 15 mm Hg ) before and after production of diffuse ischemic left ventricular dysfunction .
	manualset3
267228	4	426809	16	NULL	NULL	NULL	NULL	graded cardiac tamponade	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Echocardiographic and hemodynamic data were measured in closed-chest dogs during graded cardiac tamponade ( pericardial pressure 5 , 10 , and 15 mm Hg ) before and after production of diffuse ischemic left ventricular dysfunction .
	manualset3
267229	5	426809	16	NULL	NULL	NULL	NULL	pericardial pressure	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Echocardiographic and hemodynamic data were measured in closed-chest dogs during graded cardiac tamponade ( pericardial pressure 5 , 10 , and 15 mm Hg ) before and after production of diffuse ischemic left ventricular dysfunction .
	manualset3
267230	6	426809	16	NULL	NULL	NULL	NULL	5 mm Hg	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Echocardiographic and hemodynamic data were measured in closed-chest dogs during graded cardiac tamponade ( pericardial pressure 5 , 10 , and 15 mm Hg ) before and after production of diffuse ischemic left ventricular dysfunction .
	manualset3
267231	7	426809	16	NULL	NULL	NULL	NULL	10 mm Hg	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Echocardiographic and hemodynamic data were measured in closed-chest dogs during graded cardiac tamponade ( pericardial pressure 5 , 10 , and 15 mm Hg ) before and after production of diffuse ischemic left ventricular dysfunction .
	manualset3
267232	8	426809	16	NULL	NULL	NULL	NULL	production	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Echocardiographic and hemodynamic data were measured in closed-chest dogs during graded cardiac tamponade ( pericardial pressure 5 , 10 , and 15 mm Hg ) before and after production of diffuse ischemic left ventricular dysfunction .
	manualset3
267233	9	426809	16	NULL	NULL	NULL	NULL	diffuse ischemic left ventricular dysfunction	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Echocardiographic and hemodynamic data were measured in closed-chest dogs during graded cardiac tamponade ( pericardial pressure 5 , 10 , and 15 mm Hg ) before and after production of diffuse ischemic left ventricular dysfunction .
	manualset3
267234	1	426810	16	NULL	NULL	NULL	NULL	Echographic patterns	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Echographic patterns of just evolving acute pancreatitis : an experimental study .
	manualset3
267235	2	426810	16	NULL	NULL	NULL	NULL	acute pancreatitis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Echographic patterns of just evolving acute pancreatitis : an experimental study .
	manualset3
267236	3	426810	16	NULL	NULL	NULL	NULL	experimental study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Echographic patterns of just evolving acute pancreatitis : an experimental study .
	manualset3
267237	1	426811	16	NULL	NULL	NULL	NULL	Economic evaluations	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Economic evaluations in oncology will be increasingly important in making choices between expensive new treatments , but great care must be exercised in the interpretation of individual reports .
	manualset3
267238	2	426811	16	NULL	NULL	NULL	NULL	oncology	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Economic evaluations in oncology will be increasingly important in making choices between expensive new treatments , but great care must be exercised in the interpretation of individual reports .
	manualset3
267239	3	426811	16	NULL	NULL	NULL	NULL	making choices	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Economic evaluations in oncology will be increasingly important in making choices between expensive new treatments , but great care must be exercised in the interpretation of individual reports .
	manualset3
267240	4	426811	16	NULL	NULL	NULL	NULL	treatments	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Economic evaluations in oncology will be increasingly important in making choices between expensive new treatments , but great care must be exercised in the interpretation of individual reports .
	manualset3
267241	5	426811	16	NULL	NULL	NULL	NULL	care	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Economic evaluations in oncology will be increasingly important in making choices between expensive new treatments , but great care must be exercised in the interpretation of individual reports .
	manualset3
267242	6	426811	16	NULL	NULL	NULL	NULL	interpretation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Economic evaluations in oncology will be increasingly important in making choices between expensive new treatments , but great care must be exercised in the interpretation of individual reports .
	manualset3
267243	7	426811	16	NULL	NULL	NULL	NULL	individual reports	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Economic evaluations in oncology will be increasingly important in making choices between expensive new treatments , but great care must be exercised in the interpretation of individual reports .
	manualset3
267244	1	426812	16	NULL	NULL	NULL	NULL	Economists	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Economists have long been interested in measuring distributional impacts of policy interventions .
	manualset3
267245	2	426812	16	NULL	NULL	NULL	NULL	distributional impacts	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Economists have long been interested in measuring distributional impacts of policy interventions .
	manualset3
267246	3	426812	16	NULL	NULL	NULL	NULL	policy interventions	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Economists have long been interested in measuring distributional impacts of policy interventions .
	manualset3
267247	1	426813	16	NULL	NULL	NULL	NULL	Ecstasy	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ecstasy and the antecedents of illicit drug use .
	manualset3
267248	2	426813	16	NULL	NULL	NULL	NULL	antecedents	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ecstasy and the antecedents of illicit drug use .
	manualset3
267249	3	426813	16	NULL	NULL	NULL	NULL	illicit drug use	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ecstasy and the antecedents of illicit drug use .
	manualset3
267250	1	426814	16	NULL	NULL	NULL	NULL	Ectopic activation	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ectopic activation of the SIN can uncouple septum formation from other cell-cycle events , whereas loss of SIN signalling gives rise to multinucleated cells due to the failure of cytokinesis .
	manualset3
267251	2	426814	16	NULL	NULL	NULL	NULL	SIN	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ectopic activation of the SIN can uncouple septum formation from other cell-cycle events , whereas loss of SIN signalling gives rise to multinucleated cells due to the failure of cytokinesis .
	manualset3
267252	3	426814	16	NULL	NULL	NULL	NULL	septum formation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ectopic activation of the SIN can uncouple septum formation from other cell-cycle events , whereas loss of SIN signalling gives rise to multinucleated cells due to the failure of cytokinesis .
	manualset3
267253	4	426814	16	NULL	NULL	NULL	NULL	cell-cycle events	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ectopic activation of the SIN can uncouple septum formation from other cell-cycle events , whereas loss of SIN signalling gives rise to multinucleated cells due to the failure of cytokinesis .
	manualset3
267254	5	426814	16	NULL	NULL	NULL	NULL	loss	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ectopic activation of the SIN can uncouple septum formation from other cell-cycle events , whereas loss of SIN signalling gives rise to multinucleated cells due to the failure of cytokinesis .
	manualset3
267255	6	426814	16	NULL	NULL	NULL	NULL	SIN signalling	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ectopic activation of the SIN can uncouple septum formation from other cell-cycle events , whereas loss of SIN signalling gives rise to multinucleated cells due to the failure of cytokinesis .
	manualset3
267256	7	426814	16	NULL	NULL	NULL	NULL	multinucleated cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ectopic activation of the SIN can uncouple septum formation from other cell-cycle events , whereas loss of SIN signalling gives rise to multinucleated cells due to the failure of cytokinesis .
	manualset3
267257	8	426814	16	NULL	NULL	NULL	NULL	failure	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ectopic activation of the SIN can uncouple septum formation from other cell-cycle events , whereas loss of SIN signalling gives rise to multinucleated cells due to the failure of cytokinesis .
	manualset3
267258	9	426814	16	NULL	NULL	NULL	NULL	cytokinesis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ectopic activation of the SIN can uncouple septum formation from other cell-cycle events , whereas loss of SIN signalling gives rise to multinucleated cells due to the failure of cytokinesis .
	manualset3
267259	1	426815	16	NULL	NULL	NULL	NULL	Pain	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Pain and manipulation of the patient ) .
	manualset3
267260	2	426815	16	NULL	NULL	NULL	NULL	manipulation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Pain and manipulation of the patient ) .
	manualset3
267261	3	426815	16	NULL	NULL	NULL	NULL	patient	Person												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Pain and manipulation of the patient ) .
	manualset3
267262	1	426816	16	NULL	NULL	NULL	NULL	Ectopic expression	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ectopic expression coupled with pulling down analyses showed that BubR1-M was derived from SUMO modification .
	manualset3
267263	2	426816	16	NULL	NULL	NULL	NULL	pulling down analyses	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ectopic expression coupled with pulling down analyses showed that BubR1-M was derived from SUMO modification .
	manualset3
267264	3	426816	16	NULL	NULL	NULL	NULL	BubR1-M	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ectopic expression coupled with pulling down analyses showed that BubR1-M was derived from SUMO modification .
	manualset3
267265	4	426816	16	NULL	NULL	NULL	NULL	SUMO modification	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ectopic expression coupled with pulling down analyses showed that BubR1-M was derived from SUMO modification .
	manualset3
267266	1	426817	16	NULL	NULL	NULL	NULL	Ectopic expression	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ectopic expression of dMyc induces expression of Cyclin E , Cyclin D , and Cdk4 , which can inhibit Rbf and promote G ( 1 ) - S progression .
	manualset3
267267	2	426817	16	NULL	NULL	NULL	NULL	dMyc	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ectopic expression of dMyc induces expression of Cyclin E , Cyclin D , and Cdk4 , which can inhibit Rbf and promote G ( 1 ) - S progression .
	manualset3
267268	3	426817	16	NULL	NULL	NULL	NULL	expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ectopic expression of dMyc induces expression of Cyclin E , Cyclin D , and Cdk4 , which can inhibit Rbf and promote G ( 1 ) - S progression .
	manualset3
267269	4	426817	16	NULL	NULL	NULL	NULL	Cyclin E	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ectopic expression of dMyc induces expression of Cyclin E , Cyclin D , and Cdk4 , which can inhibit Rbf and promote G ( 1 ) - S progression .
	manualset3
267270	5	426817	16	NULL	NULL	NULL	NULL	Cyclin D	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ectopic expression of dMyc induces expression of Cyclin E , Cyclin D , and Cdk4 , which can inhibit Rbf and promote G ( 1 ) - S progression .
	manualset3
267271	6	426817	16	NULL	NULL	NULL	NULL	Cdk4	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ectopic expression of dMyc induces expression of Cyclin E , Cyclin D , and Cdk4 , which can inhibit Rbf and promote G ( 1 ) - S progression .
	manualset3
267272	7	426817	16	NULL	NULL	NULL	NULL	Rbf	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ectopic expression of dMyc induces expression of Cyclin E , Cyclin D , and Cdk4 , which can inhibit Rbf and promote G ( 1 ) - S progression .
	manualset3
267273	8	426817	16	NULL	NULL	NULL	NULL	G ( 1 ) - S progression	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Ectopic expression of dMyc induces expression of Cyclin E , Cyclin D , and Cdk4 , which can inhibit Rbf and promote G ( 1 ) - S progression .
	manualset3
267274	1	426818	16	NULL	NULL	NULL	NULL	Editorial	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Editorial : Dental needs and manpower resources .
	manualset3
267275	2	426818	16	NULL	NULL	NULL	NULL	Dental needs	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Editorial : Dental needs and manpower resources .
	manualset3
267276	3	426818	16	NULL	NULL	NULL	NULL	manpower resources	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Editorial : Dental needs and manpower resources .
	manualset3
267277	1	426819	16	NULL	NULL	NULL	NULL	Editorial comment	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Editorial comment on : Molecular mechanisms related to parturition-induced stress urinary incontinence .
	manualset3
267278	2	426819	16	NULL	NULL	NULL	NULL	Molecular mechanisms	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Editorial comment on : Molecular mechanisms related to parturition-induced stress urinary incontinence .
	manualset3
267279	3	426819	16	NULL	NULL	NULL	NULL	parturition-induced stress urinary incontinence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Editorial comment on : Molecular mechanisms related to parturition-induced stress urinary incontinence .
	manualset3
267280	1	426820	16	NULL	NULL	NULL	NULL	Editors	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Editors ' Strategic Implications : the authors ' focus on the public health value of a prevention strategy is compelling and provides a model for analyses of other strategies and content areas .
	manualset3
267281	2	426820	16	NULL	NULL	NULL	NULL	Strategic Implications	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Editors ' Strategic Implications : the authors ' focus on the public health value of a prevention strategy is compelling and provides a model for analyses of other strategies and content areas .
	manualset3
267282	3	426820	16	NULL	NULL	NULL	NULL	authors ' focus	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Editors ' Strategic Implications : the authors ' focus on the public health value of a prevention strategy is compelling and provides a model for analyses of other strategies and content areas .
	manualset3
267283	4	426820	16	NULL	NULL	NULL	NULL	public health value	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Editors ' Strategic Implications : the authors ' focus on the public health value of a prevention strategy is compelling and provides a model for analyses of other strategies and content areas .
	manualset3
267284	5	426820	16	NULL	NULL	NULL	NULL	prevention strategy	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Editors ' Strategic Implications : the authors ' focus on the public health value of a prevention strategy is compelling and provides a model for analyses of other strategies and content areas .
	manualset3
267285	6	426820	16	NULL	NULL	NULL	NULL	model	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Editors ' Strategic Implications : the authors ' focus on the public health value of a prevention strategy is compelling and provides a model for analyses of other strategies and content areas .
	manualset3
267286	7	426820	16	NULL	NULL	NULL	NULL	analyses	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Editors ' Strategic Implications : the authors ' focus on the public health value of a prevention strategy is compelling and provides a model for analyses of other strategies and content areas .
	manualset3
267287	8	426820	16	NULL	NULL	NULL	NULL	strategies and content areas	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Editors ' Strategic Implications : the authors ' focus on the public health value of a prevention strategy is compelling and provides a model for analyses of other strategies and content areas .
	manualset3
267288	1	426821	16	NULL	NULL	NULL	NULL	Edman degradation	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Edman degradation demonstrated 106 amino acids residues in the Col 1 and 149 residues in the Col 2 domain .
	manualset3
267289	2	426821	16	NULL	NULL	NULL	NULL	106 amino acids residues	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Edman degradation demonstrated 106 amino acids residues in the Col 1 and 149 residues in the Col 2 domain .
	manualset3
267290	3	426821	16	NULL	NULL	NULL	NULL	Col 1	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Edman degradation demonstrated 106 amino acids residues in the Col 1 and 149 residues in the Col 2 domain .
	manualset3
267291	4	426821	16	NULL	NULL	NULL	NULL	149 residues	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Edman degradation demonstrated 106 amino acids residues in the Col 1 and 149 residues in the Col 2 domain .
	manualset3
267292	5	426821	16	NULL	NULL	NULL	NULL	Col 2 domain	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Edman degradation demonstrated 106 amino acids residues in the Col 1 and 149 residues in the Col 2 domain .
	manualset3
267293	1	426822	16	NULL	NULL	NULL	NULL	primary care providers	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Educating primary care providers , including gerontological nurses , to recognize signs of substance abuse in this population and providing age-appropriate treatment options is critically important but will require funding beyond what is currently available .
	manualset3
267294	2	426822	16	NULL	NULL	NULL	NULL	gerontological nurses	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Educating primary care providers , including gerontological nurses , to recognize signs of substance abuse in this population and providing age-appropriate treatment options is critically important but will require funding beyond what is currently available .
	manualset3
267295	3	426822	16	NULL	NULL	NULL	NULL	signs	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Educating primary care providers , including gerontological nurses , to recognize signs of substance abuse in this population and providing age-appropriate treatment options is critically important but will require funding beyond what is currently available .
	manualset3
267296	4	426822	16	NULL	NULL	NULL	NULL	substance abuse	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Educating primary care providers , including gerontological nurses , to recognize signs of substance abuse in this population and providing age-appropriate treatment options is critically important but will require funding beyond what is currently available .
	manualset3
267297	5	426822	16	NULL	NULL	NULL	NULL	population	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Educating primary care providers , including gerontological nurses , to recognize signs of substance abuse in this population and providing age-appropriate treatment options is critically important but will require funding beyond what is currently available .
	manualset3
267298	6	426822	16	NULL	NULL	NULL	NULL	age-appropriate treatment options	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Educating primary care providers , including gerontological nurses , to recognize signs of substance abuse in this population and providing age-appropriate treatment options is critically important but will require funding beyond what is currently available .
	manualset3
267299	1	426823	16	NULL	NULL	NULL	NULL	3-isobutyl-1-methylxanthine	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of 3-isobutyl-1-methylxanthine on HCO3 - transport in turtle bladder .
	manualset3
267300	2	426823	16	NULL	NULL	NULL	NULL	HCO3 - transport	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of 3-isobutyl-1-methylxanthine on HCO3 - transport in turtle bladder .
	manualset3
267301	3	426823	16	NULL	NULL	NULL	NULL	turtle	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of 3-isobutyl-1-methylxanthine on HCO3 - transport in turtle bladder .
	manualset3
267302	4	426823	16	NULL	NULL	NULL	NULL	bladder	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of 3-isobutyl-1-methylxanthine on HCO3 - transport in turtle bladder .
	manualset3
267303	1	426824	16	NULL	NULL	NULL	NULL	Effect	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of 5-hydroxytryptamine precursors on morphine analgesia in the formalin test .
	manualset3
267304	2	426824	16	NULL	NULL	NULL	NULL	5-hydroxytryptamine precursors	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of 5-hydroxytryptamine precursors on morphine analgesia in the formalin test .
	manualset3
267305	3	426824	16	NULL	NULL	NULL	NULL	morphine analgesia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of 5-hydroxytryptamine precursors on morphine analgesia in the formalin test .
	manualset3
267306	4	426824	16	NULL	NULL	NULL	NULL	formalin test	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of 5-hydroxytryptamine precursors on morphine analgesia in the formalin test .
	manualset3
267307	1	426825	16	NULL	NULL	NULL	NULL	Effect	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of ACTH-challenge on progesterone and cortisol levels in ovariectomised repeat breeder heifers .
	manualset3
267308	2	426825	16	NULL	NULL	NULL	NULL	ACTH-challenge	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of ACTH-challenge on progesterone and cortisol levels in ovariectomised repeat breeder heifers .
	manualset3
267309	3	426825	16	NULL	NULL	NULL	NULL	progesterone levels	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of ACTH-challenge on progesterone and cortisol levels in ovariectomised repeat breeder heifers .
	manualset3
267310	4	426825	16	NULL	NULL	NULL	NULL	cortisol levels	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of ACTH-challenge on progesterone and cortisol levels in ovariectomised repeat breeder heifers .
	manualset3
267311	5	426825	16	NULL	NULL	NULL	NULL	ovariectomised repeat breeder heifers	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of ACTH-challenge on progesterone and cortisol levels in ovariectomised repeat breeder heifers .
	manualset3
267312	1	426826	16	NULL	NULL	NULL	NULL	Effect	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of AD-1590 , a non-steroidal anti-inflammatory agent with a potent antipyretic activity , on in vitro prostaglandin generation in rabbit brain .
	manualset3
267313	2	426826	16	NULL	NULL	NULL	NULL	AD-1590	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of AD-1590 , a non-steroidal anti-inflammatory agent with a potent antipyretic activity , on in vitro prostaglandin generation in rabbit brain .
	manualset3
267314	3	426826	16	NULL	NULL	NULL	NULL	non-steroidal anti-inflammatory agent	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of AD-1590 , a non-steroidal anti-inflammatory agent with a potent antipyretic activity , on in vitro prostaglandin generation in rabbit brain .
	manualset3
267315	4	426826	16	NULL	NULL	NULL	NULL	potent antipyretic activity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of AD-1590 , a non-steroidal anti-inflammatory agent with a potent antipyretic activity , on in vitro prostaglandin generation in rabbit brain .
	manualset3
267316	5	426826	16	NULL	NULL	NULL	NULL	in vitro prostaglandin generation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of AD-1590 , a non-steroidal anti-inflammatory agent with a potent antipyretic activity , on in vitro prostaglandin generation in rabbit brain .
	manualset3
267317	6	426826	16	NULL	NULL	NULL	NULL	rabbit	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of AD-1590 , a non-steroidal anti-inflammatory agent with a potent antipyretic activity , on in vitro prostaglandin generation in rabbit brain .
	manualset3
267318	7	426826	16	NULL	NULL	NULL	NULL	brain	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of AD-1590 , a non-steroidal anti-inflammatory agent with a potent antipyretic activity , on in vitro prostaglandin generation in rabbit brain .
	manualset3
267319	1	426827	16	NULL	NULL	NULL	NULL	Effect	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of Ayurvedic herbs on control of plaque and gingivitis : A randomized controlled trial .
	manualset3
267320	2	426827	16	NULL	NULL	NULL	NULL	Ayurvedic herbs	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of Ayurvedic herbs on control of plaque and gingivitis : A randomized controlled trial .
	manualset3
267321	3	426827	16	NULL	NULL	NULL	NULL	control	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of Ayurvedic herbs on control of plaque and gingivitis : A randomized controlled trial .
	manualset3
267322	4	426827	16	NULL	NULL	NULL	NULL	plaque	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of Ayurvedic herbs on control of plaque and gingivitis : A randomized controlled trial .
	manualset3
267323	5	426827	16	NULL	NULL	NULL	NULL	gingivitis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of Ayurvedic herbs on control of plaque and gingivitis : A randomized controlled trial .
	manualset3
267324	6	426827	16	NULL	NULL	NULL	NULL	randomized controlled trial	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of Ayurvedic herbs on control of plaque and gingivitis : A randomized controlled trial .
	manualset3
267325	1	426828	16	NULL	NULL	NULL	NULL	Effect	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of PKC-zeta mediating Ang II-stimulated activation of CCDPK on rat cardiac fibroblast proliferation .
	manualset3
267326	2	426828	16	NULL	NULL	NULL	NULL	PKC-zeta	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of PKC-zeta mediating Ang II-stimulated activation of CCDPK on rat cardiac fibroblast proliferation .
	manualset3
267327	3	426828	16	NULL	NULL	NULL	NULL	Ang II-stimulated activation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of PKC-zeta mediating Ang II-stimulated activation of CCDPK on rat cardiac fibroblast proliferation .
	manualset3
267328	4	426828	16	NULL	NULL	NULL	NULL	CCDPK	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of PKC-zeta mediating Ang II-stimulated activation of CCDPK on rat cardiac fibroblast proliferation .
	manualset3
267329	5	426828	16	NULL	NULL	NULL	NULL	rat	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of PKC-zeta mediating Ang II-stimulated activation of CCDPK on rat cardiac fibroblast proliferation .
	manualset3
267330	6	426828	16	NULL	NULL	NULL	NULL	cardiac fibroblast proliferation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of PKC-zeta mediating Ang II-stimulated activation of CCDPK on rat cardiac fibroblast proliferation .
	manualset3
267331	1	426829	16	NULL	NULL	NULL	NULL	Effect	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of acidic and basic isoferritins on in vitro growth of human granulocyte-monocyte progenitors .
	manualset3
267332	2	426829	16	NULL	NULL	NULL	NULL	acidic and basic isoferritins	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of acidic and basic isoferritins on in vitro growth of human granulocyte-monocyte progenitors .
	manualset3
267333	3	426829	16	NULL	NULL	NULL	NULL	in vitro growth	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of acidic and basic isoferritins on in vitro growth of human granulocyte-monocyte progenitors .
	manualset3
267334	4	426829	16	NULL	NULL	NULL	NULL	human granulocyte-monocyte progenitors	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of acidic and basic isoferritins on in vitro growth of human granulocyte-monocyte progenitors .
	manualset3
267335	1	426830	16	NULL	NULL	NULL	NULL	Effect	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of acute ethanol administration on tryptophan oxygenase activity in rat liver .
	manualset3
267336	2	426830	16	NULL	NULL	NULL	NULL	acute ethanol administration	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of acute ethanol administration on tryptophan oxygenase activity in rat liver .
	manualset3
267337	3	426830	16	NULL	NULL	NULL	NULL	tryptophan oxygenase activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of acute ethanol administration on tryptophan oxygenase activity in rat liver .
	manualset3
267338	4	426830	16	NULL	NULL	NULL	NULL	rat	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of acute ethanol administration on tryptophan oxygenase activity in rat liver .
	manualset3
267339	5	426830	16	NULL	NULL	NULL	NULL	liver	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of acute ethanol administration on tryptophan oxygenase activity in rat liver .
	manualset3
267340	1	426831	16	NULL	NULL	NULL	NULL	Effect	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of acute removal of potassium from the body on tissue electrolytes .
	manualset3
267341	2	426831	16	NULL	NULL	NULL	NULL	acute removal	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of acute removal of potassium from the body on tissue electrolytes .
	manualset3
267342	3	426831	16	NULL	NULL	NULL	NULL	potassium	Ion												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of acute removal of potassium from the body on tissue electrolytes .
	manualset3
267343	4	426831	16	NULL	NULL	NULL	NULL	body	AnatomicalPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of acute removal of potassium from the body on tissue electrolytes .
	manualset3
267344	5	426831	16	NULL	NULL	NULL	NULL	tissue electrolytes	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of acute removal of potassium from the body on tissue electrolytes .
	manualset3
267345	1	426832	16	NULL	NULL	NULL	NULL	Effect	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of antigen-induced synovitis on the extensor tendons within the retinacular compartment of the dog .
	manualset3
267346	2	426832	16	NULL	NULL	NULL	NULL	antigen-induced synovitis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of antigen-induced synovitis on the extensor tendons within the retinacular compartment of the dog .
	manualset3
267347	3	426832	16	NULL	NULL	NULL	NULL	extensor tendons	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of antigen-induced synovitis on the extensor tendons within the retinacular compartment of the dog .
	manualset3
267348	4	426832	16	NULL	NULL	NULL	NULL	retinacular compartment	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of antigen-induced synovitis on the extensor tendons within the retinacular compartment of the dog .
	manualset3
267349	5	426832	16	NULL	NULL	NULL	NULL	dog	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of antigen-induced synovitis on the extensor tendons within the retinacular compartment of the dog .
	manualset3
267350	1	426833	16	NULL	NULL	NULL	NULL	Effect	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of apolipoprotein E , peroxisome proliferator-activated receptor alpha and lipoprotein lipase gene mutations on the ability of fenofibrate to improve lipid profiles and reach clinical guideline targets among hypertriglyceridemic patients .
	manualset3
267351	2	426833	16	NULL	NULL	NULL	NULL	apolipoprotein E gene mutations	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of apolipoprotein E , peroxisome proliferator-activated receptor alpha and lipoprotein lipase gene mutations on the ability of fenofibrate to improve lipid profiles and reach clinical guideline targets among hypertriglyceridemic patients .
	manualset3
267352	3	426833	16	NULL	NULL	NULL	NULL	peroxisome proliferator-activated receptor alpha gene mutations	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of apolipoprotein E , peroxisome proliferator-activated receptor alpha and lipoprotein lipase gene mutations on the ability of fenofibrate to improve lipid profiles and reach clinical guideline targets among hypertriglyceridemic patients .
	manualset3
267353	4	426833	16	NULL	NULL	NULL	NULL	lipoprotein lipase gene mutations	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of apolipoprotein E , peroxisome proliferator-activated receptor alpha and lipoprotein lipase gene mutations on the ability of fenofibrate to improve lipid profiles and reach clinical guideline targets among hypertriglyceridemic patients .
	manualset3
267354	5	426833	16	NULL	NULL	NULL	NULL	ability	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of apolipoprotein E , peroxisome proliferator-activated receptor alpha and lipoprotein lipase gene mutations on the ability of fenofibrate to improve lipid profiles and reach clinical guideline targets among hypertriglyceridemic patients .
	manualset3
267355	6	426833	16	NULL	NULL	NULL	NULL	fenofibrate	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of apolipoprotein E , peroxisome proliferator-activated receptor alpha and lipoprotein lipase gene mutations on the ability of fenofibrate to improve lipid profiles and reach clinical guideline targets among hypertriglyceridemic patients .
	manualset3
267356	7	426833	16	NULL	NULL	NULL	NULL	lipid profiles	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of apolipoprotein E , peroxisome proliferator-activated receptor alpha and lipoprotein lipase gene mutations on the ability of fenofibrate to improve lipid profiles and reach clinical guideline targets among hypertriglyceridemic patients .
	manualset3
267357	8	426833	16	NULL	NULL	NULL	NULL	clinical guideline targets	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of apolipoprotein E , peroxisome proliferator-activated receptor alpha and lipoprotein lipase gene mutations on the ability of fenofibrate to improve lipid profiles and reach clinical guideline targets among hypertriglyceridemic patients .
	manualset3
267358	9	426833	16	NULL	NULL	NULL	NULL	hypertriglyceridemic patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of apolipoprotein E , peroxisome proliferator-activated receptor alpha and lipoprotein lipase gene mutations on the ability of fenofibrate to improve lipid profiles and reach clinical guideline targets among hypertriglyceridemic patients .
	manualset3
267359	1	426834	16	NULL	NULL	NULL	NULL	Effect	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of arbuscular mycorrhizal ( G. etunicatum ) fungus on antioxidant enzymes activity under zinc toxicity in lettuce plants .
	manualset3
267360	2	426834	16	NULL	NULL	NULL	NULL	arbuscular mycorrhizal ( G. etunicatum ) fungus	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of arbuscular mycorrhizal ( G. etunicatum ) fungus on antioxidant enzymes activity under zinc toxicity in lettuce plants .
	manualset3
267361	3	426834	16	NULL	NULL	NULL	NULL	antioxidant enzymes activity	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of arbuscular mycorrhizal ( G. etunicatum ) fungus on antioxidant enzymes activity under zinc toxicity in lettuce plants .
	manualset3
267362	4	426834	16	NULL	NULL	NULL	NULL	zinc toxicity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of arbuscular mycorrhizal ( G. etunicatum ) fungus on antioxidant enzymes activity under zinc toxicity in lettuce plants .
	manualset3
267363	5	426834	16	NULL	NULL	NULL	NULL	lettuce plants	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of arbuscular mycorrhizal ( G. etunicatum ) fungus on antioxidant enzymes activity under zinc toxicity in lettuce plants .
	manualset3
267364	1	426835	16	NULL	NULL	NULL	NULL	Effect	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of centralized intake on outcomes of substance abuse treatment .
	manualset3
267365	2	426835	16	NULL	NULL	NULL	NULL	centralized intake	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of centralized intake on outcomes of substance abuse treatment .
	manualset3
267366	3	426835	16	NULL	NULL	NULL	NULL	outcomes	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of centralized intake on outcomes of substance abuse treatment .
	manualset3
267367	4	426835	16	NULL	NULL	NULL	NULL	substance abuse treatment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of centralized intake on outcomes of substance abuse treatment .
	manualset3
267368	1	426836	16	NULL	NULL	NULL	NULL	Effect	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of chlorpromazine and reserpine on the central actions of morphine in the cat .
	manualset3
267369	2	426836	16	NULL	NULL	NULL	NULL	chlorpromazine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of chlorpromazine and reserpine on the central actions of morphine in the cat .
	manualset3
267370	3	426836	16	NULL	NULL	NULL	NULL	reserpine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of chlorpromazine and reserpine on the central actions of morphine in the cat .
	manualset3
267371	4	426836	16	NULL	NULL	NULL	NULL	central actions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of chlorpromazine and reserpine on the central actions of morphine in the cat .
	manualset3
267372	5	426836	16	NULL	NULL	NULL	NULL	morphine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of chlorpromazine and reserpine on the central actions of morphine in the cat .
	manualset3
267373	6	426836	16	NULL	NULL	NULL	NULL	cat	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of chlorpromazine and reserpine on the central actions of morphine in the cat .
	manualset3
267374	1	426837	16	NULL	NULL	NULL	NULL	Effect	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of cholesterol lowering treatment on positive exercise tests in patients with hypercholesterolemia and normal coronary angiograms .
	manualset3
267375	2	426837	16	NULL	NULL	NULL	NULL	cholesterol lowering treatment	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of cholesterol lowering treatment on positive exercise tests in patients with hypercholesterolemia and normal coronary angiograms .
	manualset3
267376	3	426837	16	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of cholesterol lowering treatment on positive exercise tests in patients with hypercholesterolemia and normal coronary angiograms .
	manualset3
267377	4	426837	16	NULL	NULL	NULL	NULL	hypercholesterolemia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of cholesterol lowering treatment on positive exercise tests in patients with hypercholesterolemia and normal coronary angiograms .
	manualset3
267378	5	426837	16	NULL	NULL	NULL	NULL	normal coronary angiograms	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Effect of cholesterol lowering treatment on positive exercise tests in patients with hypercholesterolemia and normal coronary angiograms .
	manualset3
230409	1	427831	16	NULL	NULL	0	NULL	Sema3A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Following exposure to Sema3A , PTEN accumulates rapidly at the growth cone membrane suggesting a mechanism by which PTEN couples Sema3A signalling to growth cone collapse .
	manualset3
230414	2	427831	16	NULL	NULL	0	NULL	PTEN	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Following exposure to Sema3A , PTEN accumulates rapidly at the growth cone membrane suggesting a mechanism by which PTEN couples Sema3A signalling to growth cone collapse .
	manualset3
230421	3	427831	16	NULL	NULL	0	NULL	Growth cone membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Following exposure to Sema3A , PTEN accumulates rapidly at the growth cone membrane suggesting a mechanism by which PTEN couples Sema3A signalling to growth cone collapse .
	manualset3
230526	4	427831	16	NULL	NULL	0	NULL	mechanism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Following exposure to Sema3A , PTEN accumulates rapidly at the growth cone membrane suggesting a mechanism by which PTEN couples Sema3A signalling to growth cone collapse .
	manualset3
230536	5	427831	16	NULL	NULL	0	NULL	PTEN	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Following exposure to Sema3A , PTEN accumulates rapidly at the growth cone membrane suggesting a mechanism by which PTEN couples Sema3A signalling to growth cone collapse .
	manualset3
230540	6	427831	16	NULL	NULL	0	NULL	Sem3A	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Following exposure to Sema3A , PTEN accumulates rapidly at the growth cone membrane suggesting a mechanism by which PTEN couples Sema3A signalling to growth cone collapse .
	manualset3
230543	7	427831	16	NULL	NULL	0	NULL	Sem3A signaling	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Following exposure to Sema3A , PTEN accumulates rapidly at the growth cone membrane suggesting a mechanism by which PTEN couples Sema3A signalling to growth cone collapse .
	manualset3
230544	8	427831	16	NULL	NULL	0	NULL	growth cone collapse	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Following exposure to Sema3A , PTEN accumulates rapidly at the growth cone membrane suggesting a mechanism by which PTEN couples Sema3A signalling to growth cone collapse .
	manualset3
234646	9	427831	16	NULL	NULL	NULL	NULL	exposure	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following exposure to Sema3A , PTEN accumulates rapidly at the growth cone membrane suggesting a mechanism by which PTEN couples Sema3A signalling to growth cone collapse .
	manualset3
230546	1	427832	16	NULL	NULL	0	NULL	extraction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Following extraction , gas-liquid chromatography was used to separate doxapram from basic metabolites .
	manualset3
230548	2	427832	16	NULL	NULL	0	NULL	gas-liquid chromatography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Following extraction , gas-liquid chromatography was used to separate doxapram from basic metabolites .
	manualset3
230549	3	427832	16	NULL	NULL	0	NULL	doxapram	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Following extraction , gas-liquid chromatography was used to separate doxapram from basic metabolites .
	manualset3
230752	4	427832	16	NULL	NULL	0	NULL	basic metabolites	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Following extraction , gas-liquid chromatography was used to separate doxapram from basic metabolites .
	manualset3
230554	1	427833	16	NULL	NULL	NULL	NULL	induction	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following induction of vitellogenin synthesis in the liver , liver somatic index ( LSI ) rose from 1.25 to 2.00 in 14 days .
	manualset3
230556	2	427833	16	NULL	NULL	NULL	NULL	vitellogenin synthesis	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following induction of vitellogenin synthesis in the liver , liver somatic index ( LSI ) rose from 1.25 to 2.00 in 14 days .
	manualset3
230558	3	427833	16	NULL	NULL	NULL	NULL	liver somatic index ( LSI )	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following induction of vitellogenin synthesis in the liver , liver somatic index ( LSI ) rose from 1.25 to 2.00 in 14 days .
	manualset3
230756	4	427833	16	NULL	NULL	0	NULL	rose from 1.25 to 2.00	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Following induction of vitellogenin synthesis in the liver , liver somatic index ( LSI ) rose from 1.25 to 2.00 in 14 days .
	manualset3
230757	5	427833	16	NULL	NULL	0	NULL	14 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Following induction of vitellogenin synthesis in the liver , liver somatic index ( LSI ) rose from 1.25 to 2.00 in 14 days .
	manualset3
235774	6	427833	16	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Following induction of vitellogenin synthesis in the liver , liver somatic index ( LSI ) rose from 1.25 to 2.00 in 14 days .
	manualset3
230563	1	427834	16	NULL	NULL	0	NULL	change in recruitment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Recent change in recruitment and statute of physicians of hospitals of the second category ) .
	manualset3
230564	2	427834	16	NULL	NULL	0	NULL	statute of physicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Recent change in recruitment and statute of physicians of hospitals of the second category ) .
	manualset3
230565	3	427834	16	NULL	NULL	0	NULL	hospitals of the second category	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( Recent change in recruitment and statute of physicians of hospitals of the second category ) .
	manualset3
230566	1	427835	16	NULL	NULL	0	NULL	round-the-clock therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Following intensive round-the-clock therapy with theophylline ( the dosage of which maintained serum levels of theophylline between 10 microgram/ml and 20 microgram/ml ) and therapy with prednisone ( 20 mg twice daily for three weeks or more ) , there were improvements in spirometric and body plethysmographic measurements .
	manualset3
230567	2	427835	16	NULL	NULL	0	NULL	theophylline	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Following intensive round-the-clock therapy with theophylline ( the dosage of which maintained serum levels of theophylline between 10 microgram/ml and 20 microgram/ml ) and therapy with prednisone ( 20 mg twice daily for three weeks or more ) , there were improvements in spirometric and body plethysmographic measurements .
	manualset3
230568	3	427835	16	NULL	NULL	NULL	NULL	dosage	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following intensive round-the-clock therapy with theophylline ( the dosage of which maintained serum levels of theophylline between 10 microgram/ml and 20 microgram/ml ) and therapy with prednisone ( 20 mg twice daily for three weeks or more ) , there were improvements in spirometric and body plethysmographic measurements .
	manualset3
234874	4	427835	16	NULL	NULL	0	NULL	serum levels	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Following intensive round-the-clock therapy with theophylline ( the dosage of which maintained serum levels of theophylline between 10 microgram/ml and 20 microgram/ml ) and therapy with prednisone ( 20 mg twice daily for three weeks or more ) , there were improvements in spirometric and body plethysmographic measurements .
	manualset3
234875	5	427835	16	NULL	NULL	0	NULL	theophylline	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Following intensive round-the-clock therapy with theophylline ( the dosage of which maintained serum levels of theophylline between 10 microgram/ml and 20 microgram/ml ) and therapy with prednisone ( 20 mg twice daily for three weeks or more ) , there were improvements in spirometric and body plethysmographic measurements .
	manualset3
234876	6	427835	16	NULL	NULL	0	NULL	10 microgram/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Following intensive round-the-clock therapy with theophylline ( the dosage of which maintained serum levels of theophylline between 10 microgram/ml and 20 microgram/ml ) and therapy with prednisone ( 20 mg twice daily for three weeks or more ) , there were improvements in spirometric and body plethysmographic measurements .
	manualset3
234877	7	427835	16	NULL	NULL	0	NULL	20 microgram/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Following intensive round-the-clock therapy with theophylline ( the dosage of which maintained serum levels of theophylline between 10 microgram/ml and 20 microgram/ml ) and therapy with prednisone ( 20 mg twice daily for three weeks or more ) , there were improvements in spirometric and body plethysmographic measurements .
	manualset3
234878	8	427835	16	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Following intensive round-the-clock therapy with theophylline ( the dosage of which maintained serum levels of theophylline between 10 microgram/ml and 20 microgram/ml ) and therapy with prednisone ( 20 mg twice daily for three weeks or more ) , there were improvements in spirometric and body plethysmographic measurements .
	manualset3
234879	9	427835	16	NULL	NULL	0	NULL	prednisone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Following intensive round-the-clock therapy with theophylline ( the dosage of which maintained serum levels of theophylline between 10 microgram/ml and 20 microgram/ml ) and therapy with prednisone ( 20 mg twice daily for three weeks or more ) , there were improvements in spirometric and body plethysmographic measurements .
	manualset3
234880	10	427835	16	NULL	NULL	0	NULL	20 mg 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Following intensive round-the-clock therapy with theophylline ( the dosage of which maintained serum levels of theophylline between 10 microgram/ml and 20 microgram/ml ) and therapy with prednisone ( 20 mg twice daily for three weeks or more ) , there were improvements in spirometric and body plethysmographic measurements .
	manualset3
234881	11	427835	16	NULL	NULL	0	NULL	three weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Following intensive round-the-clock therapy with theophylline ( the dosage of which maintained serum levels of theophylline between 10 microgram/ml and 20 microgram/ml ) and therapy with prednisone ( 20 mg twice daily for three weeks or more ) , there were improvements in spirometric and body plethysmographic measurements .
	manualset3
234882	12	427835	16	NULL	NULL	0	NULL	improvements	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Following intensive round-the-clock therapy with theophylline ( the dosage of which maintained serum levels of theophylline between 10 microgram/ml and 20 microgram/ml ) and therapy with prednisone ( 20 mg twice daily for three weeks or more ) , there were improvements in spirometric and body plethysmographic measurements .
	manualset3
234883	13	427835	16	NULL	NULL	0	NULL	spirometric measurements	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Following intensive round-the-clock therapy with theophylline ( the dosage of which maintained serum levels of theophylline between 10 microgram/ml and 20 microgram/ml ) and therapy with prednisone ( 20 mg twice daily for three weeks or more ) , there were improvements in spirometric and body plethysmographic measurements .
	manualset3
234884	14	427835	16	NULL	NULL	0	NULL	body plethysmographic measurements	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Following intensive round-the-clock therapy with theophylline ( the dosage of which maintained serum levels of theophylline between 10 microgram/ml and 20 microgram/ml ) and therapy with prednisone ( 20 mg twice daily for three weeks or more ) , there were improvements in spirometric and body plethysmographic measurements .
	manualset3
230574	1	427836	16	NULL	NULL	NULL	NULL	oral infection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following oral infection of Microtus agrestis with sporocysts of Frenkelia microti , transient focal necrosis and cellular infiltrations in the liver , hyperplasia of lymphoid organs , and inflammatory infiltrations in the heart , pulmonary veins , skeletal muscles and brain occurred during the first asexual multiplication period of the parasite in the liver .
	manualset3
230575	2	427836	16	NULL	NULL	0	NULL	Microtus agrestis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Following oral infection of Microtus agrestis with sporocysts of Frenkelia microti , transient focal necrosis and cellular infiltrations in the liver , hyperplasia of lymphoid organs , and inflammatory infiltrations in the heart , pulmonary veins , skeletal muscles and brain occurred during the first asexual multiplication period of the parasite in the liver .
	manualset3
230576	3	427836	16	NULL	NULL	0	NULL	sporocysts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Following oral infection of Microtus agrestis with sporocysts of Frenkelia microti , transient focal necrosis and cellular infiltrations in the liver , hyperplasia of lymphoid organs , and inflammatory infiltrations in the heart , pulmonary veins , skeletal muscles and brain occurred during the first asexual multiplication period of the parasite in the liver .
	manualset3
230577	4	427836	16	NULL	NULL	0	NULL	Frenkelia microti	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Following oral infection of Microtus agrestis with sporocysts of Frenkelia microti , transient focal necrosis and cellular infiltrations in the liver , hyperplasia of lymphoid organs , and inflammatory infiltrations in the heart , pulmonary veins , skeletal muscles and brain occurred during the first asexual multiplication period of the parasite in the liver .
	manualset3
230578	5	427836	16	NULL	NULL	0	NULL	transient focal necrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Following oral infection of Microtus agrestis with sporocysts of Frenkelia microti , transient focal necrosis and cellular infiltrations in the liver , hyperplasia of lymphoid organs , and inflammatory infiltrations in the heart , pulmonary veins , skeletal muscles and brain occurred during the first asexual multiplication period of the parasite in the liver .
	manualset3
230579	6	427836	16	NULL	NULL	0	NULL	cellular infiltrations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Following oral infection of Microtus agrestis with sporocysts of Frenkelia microti , transient focal necrosis and cellular infiltrations in the liver , hyperplasia of lymphoid organs , and inflammatory infiltrations in the heart , pulmonary veins , skeletal muscles and brain occurred during the first asexual multiplication period of the parasite in the liver .
	manualset3
230580	7	427836	16	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Following oral infection of Microtus agrestis with sporocysts of Frenkelia microti , transient focal necrosis and cellular infiltrations in the liver , hyperplasia of lymphoid organs , and inflammatory infiltrations in the heart , pulmonary veins , skeletal muscles and brain occurred during the first asexual multiplication period of the parasite in the liver .
	manualset3
230581	8	427836	16	NULL	NULL	0	NULL	hyperplasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Following oral infection of Microtus agrestis with sporocysts of Frenkelia microti , transient focal necrosis and cellular infiltrations in the liver , hyperplasia of lymphoid organs , and inflammatory infiltrations in the heart , pulmonary veins , skeletal muscles and brain occurred during the first asexual multiplication period of the parasite in the liver .
	manualset3
230582	9	427836	16	NULL	NULL	0	NULL	lymphoid organs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Following oral infection of Microtus agrestis with sporocysts of Frenkelia microti , transient focal necrosis and cellular infiltrations in the liver , hyperplasia of lymphoid organs , and inflammatory infiltrations in the heart , pulmonary veins , skeletal muscles and brain occurred during the first asexual multiplication period of the parasite in the liver .
	manualset3
230583	10	427836	16	NULL	NULL	0	NULL	inflammatory infiltrations	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Following oral infection of Microtus agrestis with sporocysts of Frenkelia microti , transient focal necrosis and cellular infiltrations in the liver , hyperplasia of lymphoid organs , and inflammatory infiltrations in the heart , pulmonary veins , skeletal muscles and brain occurred during the first asexual multiplication period of the parasite in the liver .
	manualset3
230584	11	427836	16	NULL	NULL	0	NULL	heart	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Following oral infection of Microtus agrestis with sporocysts of Frenkelia microti , transient focal necrosis and cellular infiltrations in the liver , hyperplasia of lymphoid organs , and inflammatory infiltrations in the heart , pulmonary veins , skeletal muscles and brain occurred during the first asexual multiplication period of the parasite in the liver .
	manualset3
230585	12	427836	16	NULL	NULL	0	NULL	pulmonary veins	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Following oral infection of Microtus agrestis with sporocysts of Frenkelia microti , transient focal necrosis and cellular infiltrations in the liver , hyperplasia of lymphoid organs , and inflammatory infiltrations in the heart , pulmonary veins , skeletal muscles and brain occurred during the first asexual multiplication period of the parasite in the liver .
	manualset3
230586	13	427836	16	NULL	NULL	0	NULL	skeletal muscles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Following oral infection of Microtus agrestis with sporocysts of Frenkelia microti , transient focal necrosis and cellular infiltrations in the liver , hyperplasia of lymphoid organs , and inflammatory infiltrations in the heart , pulmonary veins , skeletal muscles and brain occurred during the first asexual multiplication period of the parasite in the liver .
	manualset3
230587	14	427836	16	NULL	NULL	0	NULL	brain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Following oral infection of Microtus agrestis with sporocysts of Frenkelia microti , transient focal necrosis and cellular infiltrations in the liver , hyperplasia of lymphoid organs , and inflammatory infiltrations in the heart , pulmonary veins , skeletal muscles and brain occurred during the first asexual multiplication period of the parasite in the liver .
	manualset3
230588	15	427836	16	NULL	NULL	0	NULL	 asexual multiplication period	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Following oral infection of Microtus agrestis with sporocysts of Frenkelia microti , transient focal necrosis and cellular infiltrations in the liver , hyperplasia of lymphoid organs , and inflammatory infiltrations in the heart , pulmonary veins , skeletal muscles and brain occurred during the first asexual multiplication period of the parasite in the liver .
	manualset3
230589	16	427836	16	NULL	NULL	0	NULL	parasite	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Following oral infection of Microtus agrestis with sporocysts of Frenkelia microti , transient focal necrosis and cellular infiltrations in the liver , hyperplasia of lymphoid organs , and inflammatory infiltrations in the heart , pulmonary veins , skeletal muscles and brain occurred during the first asexual multiplication period of the parasite in the liver .
	manualset3
230590	17	427836	16	NULL	NULL	0	NULL	liver	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Following oral infection of Microtus agrestis with sporocysts of Frenkelia microti , transient focal necrosis and cellular infiltrations in the liver , hyperplasia of lymphoid organs , and inflammatory infiltrations in the heart , pulmonary veins , skeletal muscles and brain occurred during the first asexual multiplication period of the parasite in the liver .
	manualset3
230591	1	427837	16	NULL	NULL	NULL	NULL	exposures	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following repeated exposures of rabbits to inhalation of pneumococci , the type specific response , evidenced by type specific protective antibodies and agglutinins , varies in direct proportion to the virulence of the culture used .
	manualset3
230610	2	427837	16	NULL	NULL	0	NULL	rabbits	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Following repeated exposures of rabbits to inhalation of pneumococci , the type specific response , evidenced by type specific protective antibodies and agglutinins , varies in direct proportion to the virulence of the culture used .
	manualset3
230613	3	427837	16	NULL	NULL	NULL	NULL	inhalation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following repeated exposures of rabbits to inhalation of pneumococci , the type specific response , evidenced by type specific protective antibodies and agglutinins , varies in direct proportion to the virulence of the culture used .
	manualset3
230758	4	427837	16	NULL	NULL	NULL	NULL	pneumococci	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following repeated exposures of rabbits to inhalation of pneumococci , the type specific response , evidenced by type specific protective antibodies and agglutinins , varies in direct proportion to the virulence of the culture used .
	manualset3
230759	5	427837	16	NULL	NULL	NULL	NULL	type specific response	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following repeated exposures of rabbits to inhalation of pneumococci , the type specific response , evidenced by type specific protective antibodies and agglutinins , varies in direct proportion to the virulence of the culture used .
	manualset3
230760	6	427837	16	NULL	NULL	NULL	NULL	type specific protective antibodies	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following repeated exposures of rabbits to inhalation of pneumococci , the type specific response , evidenced by type specific protective antibodies and agglutinins , varies in direct proportion to the virulence of the culture used .
	manualset3
230761	7	427837	16	NULL	NULL	NULL	NULL	agglutinins	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following repeated exposures of rabbits to inhalation of pneumococci , the type specific response , evidenced by type specific protective antibodies and agglutinins , varies in direct proportion to the virulence of the culture used .
	manualset3
230762	8	427837	16	NULL	NULL	NULL	NULL	direct proportion	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following repeated exposures of rabbits to inhalation of pneumococci , the type specific response , evidenced by type specific protective antibodies and agglutinins , varies in direct proportion to the virulence of the culture used .
	manualset3
235790	9	427837	16	NULL	NULL	NULL	NULL	virulence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following repeated exposures of rabbits to inhalation of pneumococci , the type specific response , evidenced by type specific protective antibodies and agglutinins , varies in direct proportion to the virulence of the culture used .
	manualset3
235791	10	427837	16	NULL	NULL	0	NULL	culture	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Following repeated exposures of rabbits to inhalation of pneumococci , the type specific response , evidenced by type specific protective antibodies and agglutinins , varies in direct proportion to the virulence of the culture used .
	manualset3
230594	1	427838	16	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Following surgery , acute paraplegia was diagnosed , with a spinal cord lesion at the high thoracic level .
	manualset3
230595	2	427838	16	NULL	NULL	NULL	NULL	acute paraplegia	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following surgery , acute paraplegia was diagnosed , with a spinal cord lesion at the high thoracic level .
	manualset3
230596	3	427838	16	NULL	NULL	NULL	NULL	spinal cord lesion	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following surgery , acute paraplegia was diagnosed , with a spinal cord lesion at the high thoracic level .
	manualset3
230597	4	427838	16	NULL	NULL	NULL	NULL	 high thoracic level	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following surgery , acute paraplegia was diagnosed , with a spinal cord lesion at the high thoracic level .
	manualset3
230598	1	427839	16	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Following surgery , the patient regained consciousness and blood ammonia levels became normal .
	manualset3
230600	2	427839	16	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Following surgery , the patient regained consciousness and blood ammonia levels became normal .
	manualset3
230601	3	427839	16	NULL	NULL	NULL	NULL	consciousness	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following surgery , the patient regained consciousness and blood ammonia levels became normal .
	manualset3
230603	5	427839	16	NULL	NULL	NULL	NULL	blood ammonia levels	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following surgery , the patient regained consciousness and blood ammonia levels became normal .
	manualset3
230918	1	427840	16	NULL	NULL	0	NULL	3-week withdrawal period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the 3-week withdrawal period , immunoblotting revealed increased GFAP expression in the prefrontal cortex ( PFC ) and in the shell and core compartments of the nucleus accumbens ( NAshell and NAcore ) .
	manualset3
230919	2	427840	16	NULL	NULL	0	NULL	immunoblotting	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the 3-week withdrawal period , immunoblotting revealed increased GFAP expression in the prefrontal cortex ( PFC ) and in the shell and core compartments of the nucleus accumbens ( NAshell and NAcore ) .
	manualset3
230920	3	427840	16	NULL	NULL	NULL	NULL	GFAP expression	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following the 3-week withdrawal period , immunoblotting revealed increased GFAP expression in the prefrontal cortex ( PFC ) and in the shell and core compartments of the nucleus accumbens ( NAshell and NAcore ) .
	manualset3
230921	4	427840	16	NULL	NULL	NULL	NULL	prefrontal cortex ( PFC )	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following the 3-week withdrawal period , immunoblotting revealed increased GFAP expression in the prefrontal cortex ( PFC ) and in the shell and core compartments of the nucleus accumbens ( NAshell and NAcore ) .
	manualset3
230922	5	427840	16	NULL	NULL	NULL	NULL	shell and core compartments	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following the 3-week withdrawal period , immunoblotting revealed increased GFAP expression in the prefrontal cortex ( PFC ) and in the shell and core compartments of the nucleus accumbens ( NAshell and NAcore ) .
	manualset3
235792	6	427840	16	NULL	NULL	0	NULL	nucleus accumbens	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the 3-week withdrawal period , immunoblotting revealed increased GFAP expression in the prefrontal cortex ( PFC ) and in the shell and core compartments of the nucleus accumbens ( NAshell and NAcore ) .
	manualset3
235793	7	427840	16	NULL	NULL	0	NULL	NAshell and NAcore	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the 3-week withdrawal period , immunoblotting revealed increased GFAP expression in the prefrontal cortex ( PFC ) and in the shell and core compartments of the nucleus accumbens ( NAshell and NAcore ) .
	manualset3
230923	1	427841	16	NULL	NULL	0	NULL	challenge infections	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the challenge infections , the first-season calves developed clinical parasitic gastroenteritis , whereas the second-season heifers showed no symptoms .
	manualset3
230924	2	427841	16	NULL	NULL	0	NULL	first-season	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the challenge infections , the first-season calves developed clinical parasitic gastroenteritis , whereas the second-season heifers showed no symptoms .
	manualset3
230925	3	427841	16	NULL	NULL	0	NULL	calves	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the challenge infections , the first-season calves developed clinical parasitic gastroenteritis , whereas the second-season heifers showed no symptoms .
	manualset3
230926	4	427841	16	NULL	NULL	0	NULL	parasitic gastroenteritis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the challenge infections , the first-season calves developed clinical parasitic gastroenteritis , whereas the second-season heifers showed no symptoms .
	manualset3
230927	5	427841	16	NULL	NULL	0	NULL	second-season	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the challenge infections , the first-season calves developed clinical parasitic gastroenteritis , whereas the second-season heifers showed no symptoms .
	manualset3
230928	6	427841	16	NULL	NULL	0	NULL	heifers	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the challenge infections , the first-season calves developed clinical parasitic gastroenteritis , whereas the second-season heifers showed no symptoms .
	manualset3
230929	7	427841	16	NULL	NULL	0	NULL	no symptoms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the challenge infections , the first-season calves developed clinical parasitic gastroenteritis , whereas the second-season heifers showed no symptoms .
	manualset3
231063	1	427842	16	NULL	NULL	NULL	NULL	demonstration	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following the demonstration of onchocercal skin disease 's ( OSD ) public health and social importance in 1994 , the UNDP/World Bank/WHO Special Program for Research and Training in Tropical Diseases ( TDR ) Task Force on Onchocerciasis Operational Research was asked to assess its economic impact .
	manualset3
231064	2	427842	16	NULL	NULL	NULL	NULL	onchocercal skin disease 's ( OSD )	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following the demonstration of onchocercal skin disease 's ( OSD ) public health and social importance in 1994 , the UNDP/World Bank/WHO Special Program for Research and Training in Tropical Diseases ( TDR ) Task Force on Onchocerciasis Operational Research was asked to assess its economic impact .
	manualset3
236585	3	427842	16	NULL	NULL	0	NULL	public health	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the demonstration of onchocercal skin disease 's ( OSD ) public health and social importance in 1994 , the UNDP/World Bank/WHO Special Program for Research and Training in Tropical Diseases ( TDR ) Task Force on Onchocerciasis Operational Research was asked to assess its economic impact .
	manualset3
236586	4	427842	16	NULL	NULL	0	NULL	social importance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the demonstration of onchocercal skin disease 's ( OSD ) public health and social importance in 1994 , the UNDP/World Bank/WHO Special Program for Research and Training in Tropical Diseases ( TDR ) Task Force on Onchocerciasis Operational Research was asked to assess its economic impact .
	manualset3
236587	5	427842	16	NULL	NULL	0	NULL	1994	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the demonstration of onchocercal skin disease 's ( OSD ) public health and social importance in 1994 , the UNDP/World Bank/WHO Special Program for Research and Training in Tropical Diseases ( TDR ) Task Force on Onchocerciasis Operational Research was asked to assess its economic impact .
	manualset3
236588	6	427842	16	NULL	NULL	0	NULL	 UNDP/World Bank/WHO Special Program for Research and Training in Tropical Diseases ( TDR ) Task Force on Onchocerciasis Operational Research	PublishedSourceOfInformation												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the demonstration of onchocercal skin disease 's ( OSD ) public health and social importance in 1994 , the UNDP/World Bank/WHO Special Program for Research and Training in Tropical Diseases ( TDR ) Task Force on Onchocerciasis Operational Research was asked to assess its economic impact .
	manualset3
236589	7	427842	16	NULL	NULL	0	NULL	economic impact	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the demonstration of onchocercal skin disease 's ( OSD ) public health and social importance in 1994 , the UNDP/World Bank/WHO Special Program for Research and Training in Tropical Diseases ( TDR ) Task Force on Onchocerciasis Operational Research was asked to assess its economic impact .
	manualset3
231066	1	427843	16	NULL	NULL	NULL	NULL	removal	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following the removal of a pheochromocytoma in three female patients the daily excretion of catecholamines and their metabolites was still considerably elevated for about one week .
	manualset3
231067	2	427843	16	NULL	NULL	NULL	NULL	pheochromocytoma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following the removal of a pheochromocytoma in three female patients the daily excretion of catecholamines and their metabolites was still considerably elevated for about one week .
	manualset3
231725	3	427843	16	NULL	NULL	NULL	NULL	three female patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following the removal of a pheochromocytoma in three female patients the daily excretion of catecholamines and their metabolites was still considerably elevated for about one week .
	manualset3
231754	4	427843	16	NULL	NULL	NULL	NULL	excretion	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following the removal of a pheochromocytoma in three female patients the daily excretion of catecholamines and their metabolites was still considerably elevated for about one week .
	manualset3
231758	5	427843	16	NULL	NULL	NULL	NULL	catecholamines	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following the removal of a pheochromocytoma in three female patients the daily excretion of catecholamines and their metabolites was still considerably elevated for about one week .
	manualset3
235796	6	427843	16	NULL	NULL	0	NULL	metabolites	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the removal of a pheochromocytoma in three female patients the daily excretion of catecholamines and their metabolites was still considerably elevated for about one week .
	manualset3
235797	7	427843	16	NULL	NULL	0	NULL	one week	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Following the removal of a pheochromocytoma in three female patients the daily excretion of catecholamines and their metabolites was still considerably elevated for about one week .
	manualset3
231761	1	427844	16	NULL	NULL	0	NULL	total ischemia	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Following total ischemia all experiments showed a period with reactive hyperemia , and both duration of hyperemia and excess flow was related to the duration of the ischemia .
	manualset3
231762	2	427844	16	NULL	NULL	0	NULL	experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Following total ischemia all experiments showed a period with reactive hyperemia , and both duration of hyperemia and excess flow was related to the duration of the ischemia .
	manualset3
231763	3	427844	16	NULL	NULL	0	NULL	period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Following total ischemia all experiments showed a period with reactive hyperemia , and both duration of hyperemia and excess flow was related to the duration of the ischemia .
	manualset3
231764	4	427844	16	NULL	NULL	0	NULL	reactive hyperemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Following total ischemia all experiments showed a period with reactive hyperemia , and both duration of hyperemia and excess flow was related to the duration of the ischemia .
	manualset3
231765	5	427844	16	NULL	NULL	0	NULL	duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Following total ischemia all experiments showed a period with reactive hyperemia , and both duration of hyperemia and excess flow was related to the duration of the ischemia .
	manualset3
231766	6	427844	16	NULL	NULL	0	NULL	hyperemia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Following total ischemia all experiments showed a period with reactive hyperemia , and both duration of hyperemia and excess flow was related to the duration of the ischemia .
	manualset3
231767	7	427844	16	NULL	NULL	NULL	NULL	excess flow	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following total ischemia all experiments showed a period with reactive hyperemia , and both duration of hyperemia and excess flow was related to the duration of the ischemia .
	manualset3
231768	8	427844	16	NULL	NULL	0	NULL	duration	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Following total ischemia all experiments showed a period with reactive hyperemia , and both duration of hyperemia and excess flow was related to the duration of the ischemia .
	manualset3
231769	9	427844	16	NULL	NULL	0	NULL	ischemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Following total ischemia all experiments showed a period with reactive hyperemia , and both duration of hyperemia and excess flow was related to the duration of the ischemia .
	manualset3
231068	1	427845	16	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Following treatment for arthralgia using low doses of systemic steroid , the effects of cyclosporin combined with topical steroids was seen to alleviate dramatically the skin lesions and arthritis within 2 weeks .
	manualset3
231069	2	427845	16	NULL	NULL	0	NULL	arthralgia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Following treatment for arthralgia using low doses of systemic steroid , the effects of cyclosporin combined with topical steroids was seen to alleviate dramatically the skin lesions and arthritis within 2 weeks .
	manualset3
231070	3	427845	16	NULL	NULL	0	NULL	doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Following treatment for arthralgia using low doses of systemic steroid , the effects of cyclosporin combined with topical steroids was seen to alleviate dramatically the skin lesions and arthritis within 2 weeks .
	manualset3
231775	4	427845	16	NULL	NULL	NULL	NULL	systemic steroid	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following treatment for arthralgia using low doses of systemic steroid , the effects of cyclosporin combined with topical steroids was seen to alleviate dramatically the skin lesions and arthritis within 2 weeks .
	manualset3
231776	5	427845	16	NULL	NULL	0	NULL	cyclosporin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Following treatment for arthralgia using low doses of systemic steroid , the effects of cyclosporin combined with topical steroids was seen to alleviate dramatically the skin lesions and arthritis within 2 weeks .
	manualset3
231779	6	427845	16	NULL	NULL	NULL	NULL	topical steroids	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following treatment for arthralgia using low doses of systemic steroid , the effects of cyclosporin combined with topical steroids was seen to alleviate dramatically the skin lesions and arthritis within 2 weeks .
	manualset3
232167	8	427845	16	NULL	NULL	NULL	NULL	skin lesions	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following treatment for arthralgia using low doses of systemic steroid , the effects of cyclosporin combined with topical steroids was seen to alleviate dramatically the skin lesions and arthritis within 2 weeks .
	manualset3
232168	9	427845	16	NULL	NULL	NULL	NULL	arthritis	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Following treatment for arthralgia using low doses of systemic steroid , the effects of cyclosporin combined with topical steroids was seen to alleviate dramatically the skin lesions and arthritis within 2 weeks .
	manualset3
232256	10	427845	16	NULL	NULL	0	NULL	2 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Following treatment for arthralgia using low doses of systemic steroid , the effects of cyclosporin combined with topical steroids was seen to alleviate dramatically the skin lesions and arthritis within 2 weeks .
	manualset3
232309	1	427846	16	NULL	NULL	NULL	NULL	Food enzyme inclusion	Food												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Food enzyme inclusion improved LWG and gain : food but there was a significant wheat/enzyme interaction for gain : food with no improvement due to enzyme addition for 67 SW but a 5 % improvement for 57 SW .
	manualset3
233029	3	427846	16	NULL	NULL	0	NULL	LWG	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Food enzyme inclusion improved LWG and gain : food but there was a significant wheat/enzyme interaction for gain : food with no improvement due to enzyme addition for 67 SW but a 5 % improvement for 57 SW .
	manualset3
233030	4	427846	16	NULL	NULL	0	NULL	gain	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Food enzyme inclusion improved LWG and gain : food but there was a significant wheat/enzyme interaction for gain : food with no improvement due to enzyme addition for 67 SW but a 5 % improvement for 57 SW .
	manualset3
233031	5	427846	16	NULL	NULL	0	NULL	wheat	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Food enzyme inclusion improved LWG and gain : food but there was a significant wheat/enzyme interaction for gain : food with no improvement due to enzyme addition for 67 SW but a 5 % improvement for 57 SW .
	manualset3
233032	6	427846	16	NULL	NULL	0	NULL	enzyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Food enzyme inclusion improved LWG and gain : food but there was a significant wheat/enzyme interaction for gain : food with no improvement due to enzyme addition for 67 SW but a 5 % improvement for 57 SW .
	manualset3
233033	7	427846	16	NULL	NULL	0	NULL	gain	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Food enzyme inclusion improved LWG and gain : food but there was a significant wheat/enzyme interaction for gain : food with no improvement due to enzyme addition for 67 SW but a 5 % improvement for 57 SW .
	manualset3
233034	8	427846	16	NULL	NULL	0	NULL	Food	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Food enzyme inclusion improved LWG and gain : food but there was a significant wheat/enzyme interaction for gain : food with no improvement due to enzyme addition for 67 SW but a 5 % improvement for 57 SW .
	manualset3
233035	9	427846	16	NULL	NULL	0	NULL	enzyme	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Food enzyme inclusion improved LWG and gain : food but there was a significant wheat/enzyme interaction for gain : food with no improvement due to enzyme addition for 67 SW but a 5 % improvement for 57 SW .
	manualset3
233036	10	427846	16	NULL	NULL	0	NULL	addition	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Food enzyme inclusion improved LWG and gain : food but there was a significant wheat/enzyme interaction for gain : food with no improvement due to enzyme addition for 67 SW but a 5 % improvement for 57 SW .
	manualset3
233037	11	427846	16	NULL	NULL	0	NULL	67 SW	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Food enzyme inclusion improved LWG and gain : food but there was a significant wheat/enzyme interaction for gain : food with no improvement due to enzyme addition for 67 SW but a 5 % improvement for 57 SW .
	manualset3
233038	12	427846	16	NULL	NULL	0	NULL	5 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Food enzyme inclusion improved LWG and gain : food but there was a significant wheat/enzyme interaction for gain : food with no improvement due to enzyme addition for 67 SW but a 5 % improvement for 57 SW .
	manualset3
233039	13	427846	16	NULL	NULL	0	NULL	57 SW	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Food enzyme inclusion improved LWG and gain : food but there was a significant wheat/enzyme interaction for gain : food with no improvement due to enzyme addition for 67 SW but a 5 % improvement for 57 SW .
	manualset3
236590	14	427846	16	NULL	NULL	0	NULL	improvement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Food enzyme inclusion improved LWG and gain : food but there was a significant wheat/enzyme interaction for gain : food with no improvement due to enzyme addition for 67 SW but a 5 % improvement for 57 SW .
	manualset3
232310	1	427847	16	NULL	NULL	0	NULL	Food allergy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Food allergy and atopic eczema .
	manualset3
232311	2	427847	16	NULL	NULL	0	NULL	atopic eczema	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Food allergy and atopic eczema .
	manualset3
232312	1	427848	16	NULL	NULL	NULL	NULL	Food intake	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Food intake after gastrectomy for gastric carcinoma : the role of a gastric reservoir .
	manualset3
232313	2	427848	16	NULL	NULL	0	NULL	gastrectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Food intake after gastrectomy for gastric carcinoma : the role of a gastric reservoir .
	manualset3
232327	3	427848	16	NULL	NULL	0	NULL	gastric carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Food intake after gastrectomy for gastric carcinoma : the role of a gastric reservoir .
	manualset3
232328	4	427848	16	NULL	NULL	NULL	NULL	role	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Food intake after gastrectomy for gastric carcinoma : the role of a gastric reservoir .
	manualset3
236591	5	427848	16	NULL	NULL	0	NULL	gastric reservoir	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Food intake after gastrectomy for gastric carcinoma : the role of a gastric reservoir .
	manualset3
232460	1	427849	16	NULL	NULL	0	NULL	Recording	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Recording and prevention of injuries in a rural district ) .
	manualset3
232461	2	427849	16	NULL	NULL	0	NULL	prevention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Recording and prevention of injuries in a rural district ) .
	manualset3
232462	3	427849	16	NULL	NULL	0	NULL	injuries	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Recording and prevention of injuries in a rural district ) .
	manualset3
232520	4	427849	16	NULL	NULL	NULL	NULL	rural district	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Recording and prevention of injuries in a rural district ) .
	manualset3
232548	1	427850	16	NULL	NULL	NULL	NULL	Food restriction	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Food restriction and sex differences on concurrent , oral ethanol and water reinforcers in juvenile rhesus monkeys .
	manualset3
233395	4	427850	16	NULL	NULL	0	NULL	sex differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Food restriction and sex differences on concurrent , oral ethanol and water reinforcers in juvenile rhesus monkeys .
	manualset3
233397	6	427850	16	NULL	NULL	0	NULL	ethanol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Food restriction and sex differences on concurrent , oral ethanol and water reinforcers in juvenile rhesus monkeys .
	manualset3
233400	7	427850	16	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Food restriction and sex differences on concurrent , oral ethanol and water reinforcers in juvenile rhesus monkeys .
	manualset3
233407	8	427850	16	NULL	NULL	0	NULL	reinforcers	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Food restriction and sex differences on concurrent , oral ethanol and water reinforcers in juvenile rhesus monkeys .
	manualset3
233409	10	427850	16	NULL	NULL	NULL	NULL	juvenile rhesus monkeys	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Food restriction and sex differences on concurrent , oral ethanol and water reinforcers in juvenile rhesus monkeys .
	manualset3
233304	1	427851	16	NULL	NULL	NULL	NULL	12	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For 12 of the compounds , calculations were also conducted with the larger base sets 6-311 + G and G-311 + G. The DeltaG degrees ( acid ) values changed from 341.3 kcal/mol for CH ( 2 ) ( CO ( 2 ) Me ) ( 2 ) to 301.0 kcal/mol for PhNHC ( OH ) = C ( CN ) CH ( CF ( 3 ) ) ( 2 ) .
	manualset3
233305	2	427851	16	NULL	NULL	0	NULL	compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For 12 of the compounds , calculations were also conducted with the larger base sets 6-311 + G and G-311 + G. The DeltaG degrees ( acid ) values changed from 341.3 kcal/mol for CH ( 2 ) ( CO ( 2 ) Me ) ( 2 ) to 301.0 kcal/mol for PhNHC ( OH ) = C ( CN ) CH ( CF ( 3 ) ) ( 2 ) .
	manualset3
233306	3	427851	16	NULL	NULL	0	NULL	calculations	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For 12 of the compounds , calculations were also conducted with the larger base sets 6-311 + G and G-311 + G. The DeltaG degrees ( acid ) values changed from 341.3 kcal/mol for CH ( 2 ) ( CO ( 2 ) Me ) ( 2 ) to 301.0 kcal/mol for PhNHC ( OH ) = C ( CN ) CH ( CF ( 3 ) ) ( 2 ) .
	manualset3
236592	4	427851	16	NULL	NULL	0	NULL	base sets	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For 12 of the compounds , calculations were also conducted with the larger base sets 6-311 + G and G-311 + G. The DeltaG degrees ( acid ) values changed from 341.3 kcal/mol for CH ( 2 ) ( CO ( 2 ) Me ) ( 2 ) to 301.0 kcal/mol for PhNHC ( OH ) = C ( CN ) CH ( CF ( 3 ) ) ( 2 ) .
	manualset3
236593	5	427851	16	NULL	NULL	0	NULL	6-311 + G	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For 12 of the compounds , calculations were also conducted with the larger base sets 6-311 + G and G-311 + G. The DeltaG degrees ( acid ) values changed from 341.3 kcal/mol for CH ( 2 ) ( CO ( 2 ) Me ) ( 2 ) to 301.0 kcal/mol for PhNHC ( OH ) = C ( CN ) CH ( CF ( 3 ) ) ( 2 ) .
	manualset3
236594	6	427851	16	NULL	NULL	0	NULL	G-311 + G	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For 12 of the compounds , calculations were also conducted with the larger base sets 6-311 + G and G-311 + G. The DeltaG degrees ( acid ) values changed from 341.3 kcal/mol for CH ( 2 ) ( CO ( 2 ) Me ) ( 2 ) to 301.0 kcal/mol for PhNHC ( OH ) = C ( CN ) CH ( CF ( 3 ) ) ( 2 ) .
	manualset3
236595	7	427851	16	NULL	NULL	NULL	NULL	 DeltaG degrees ( acid )	Unit												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For 12 of the compounds , calculations were also conducted with the larger base sets 6-311 + G and G-311 + G. The DeltaG degrees ( acid ) values changed from 341.3 kcal/mol for CH ( 2 ) ( CO ( 2 ) Me ) ( 2 ) to 301.0 kcal/mol for PhNHC ( OH ) = C ( CN ) CH ( CF ( 3 ) ) ( 2 ) .
	manualset3
236596	8	427851	16	NULL	NULL	0	NULL	341.3 kcal/mol	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For 12 of the compounds , calculations were also conducted with the larger base sets 6-311 + G and G-311 + G. The DeltaG degrees ( acid ) values changed from 341.3 kcal/mol for CH ( 2 ) ( CO ( 2 ) Me ) ( 2 ) to 301.0 kcal/mol for PhNHC ( OH ) = C ( CN ) CH ( CF ( 3 ) ) ( 2 ) .
	manualset3
236597	9	427851	16	NULL	NULL	0	NULL	CH ( 2 ) ( CO ( 2 ) Me ) ( 2 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For 12 of the compounds , calculations were also conducted with the larger base sets 6-311 + G and G-311 + G. The DeltaG degrees ( acid ) values changed from 341.3 kcal/mol for CH ( 2 ) ( CO ( 2 ) Me ) ( 2 ) to 301.0 kcal/mol for PhNHC ( OH ) = C ( CN ) CH ( CF ( 3 ) ) ( 2 ) .
	manualset3
236598	10	427851	16	NULL	NULL	0	NULL	301.0 kcal/mol	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For 12 of the compounds , calculations were also conducted with the larger base sets 6-311 + G and G-311 + G. The DeltaG degrees ( acid ) values changed from 341.3 kcal/mol for CH ( 2 ) ( CO ( 2 ) Me ) ( 2 ) to 301.0 kcal/mol for PhNHC ( OH ) = C ( CN ) CH ( CF ( 3 ) ) ( 2 ) .
	manualset3
236599	11	427851	16	NULL	NULL	0	NULL	PhNHC ( OH ) = C ( CN ) CH ( CF ( 3 ) ) ( 2 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For 12 of the compounds , calculations were also conducted with the larger base sets 6-311 + G and G-311 + G. The DeltaG degrees ( acid ) values changed from 341.3 kcal/mol for CH ( 2 ) ( CO ( 2 ) Me ) ( 2 ) to 301.0 kcal/mol for PhNHC ( OH ) = C ( CN ) CH ( CF ( 3 ) ) ( 2 ) .
	manualset3
233410	1	427852	16	NULL	NULL	NULL	NULL	16-kHz tones	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For 16-kHz tones , the phase delay is up to 6pi radians over the observed cochlear length ( & lt ; 1 , 000 microm ) , and instantaneous waveforms show sound propagation along the cochlear partition , supporting the existence of the cochlear traveling wave .
	manualset3
233411	2	427852	16	NULL	NULL	NULL	NULL	phase delay	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For 16-kHz tones , the phase delay is up to 6pi radians over the observed cochlear length ( & lt ; 1 , 000 microm ) , and instantaneous waveforms show sound propagation along the cochlear partition , supporting the existence of the cochlear traveling wave .
	manualset3
233412	3	427852	16	NULL	NULL	NULL	NULL	6pi radians	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For 16-kHz tones , the phase delay is up to 6pi radians over the observed cochlear length ( & lt ; 1 , 000 microm ) , and instantaneous waveforms show sound propagation along the cochlear partition , supporting the existence of the cochlear traveling wave .
	manualset3
233414	5	427852	16	NULL	NULL	NULL	NULL	cochlear length	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For 16-kHz tones , the phase delay is up to 6pi radians over the observed cochlear length ( & lt ; 1 , 000 microm ) , and instantaneous waveforms show sound propagation along the cochlear partition , supporting the existence of the cochlear traveling wave .
	manualset3
233415	6	427852	16	NULL	NULL	0	NULL	1 , 000 microm	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For 16-kHz tones , the phase delay is up to 6pi radians over the observed cochlear length ( & lt ; 1 , 000 microm ) , and instantaneous waveforms show sound propagation along the cochlear partition , supporting the existence of the cochlear traveling wave .
	manualset3
233416	7	427852	16	NULL	NULL	NULL	NULL	waveforms	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For 16-kHz tones , the phase delay is up to 6pi radians over the observed cochlear length ( & lt ; 1 , 000 microm ) , and instantaneous waveforms show sound propagation along the cochlear partition , supporting the existence of the cochlear traveling wave .
	manualset3
233417	8	427852	16	NULL	NULL	NULL	NULL	sound propagation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For 16-kHz tones , the phase delay is up to 6pi radians over the observed cochlear length ( & lt ; 1 , 000 microm ) , and instantaneous waveforms show sound propagation along the cochlear partition , supporting the existence of the cochlear traveling wave .
	manualset3
233418	9	427852	16	NULL	NULL	0	NULL	cochlear partition	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	For 16-kHz tones , the phase delay is up to 6pi radians over the observed cochlear length ( & lt ; 1 , 000 microm ) , and instantaneous waveforms show sound propagation along the cochlear partition , supporting the existence of the cochlear traveling wave .
	manualset3
233419	10	427852	16	NULL	NULL	NULL	NULL	existence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For 16-kHz tones , the phase delay is up to 6pi radians over the observed cochlear length ( & lt ; 1 , 000 microm ) , and instantaneous waveforms show sound propagation along the cochlear partition , supporting the existence of the cochlear traveling wave .
	manualset3
237515	11	427852	16	NULL	NULL	0	NULL	cochlear traveling wave	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For 16-kHz tones , the phase delay is up to 6pi radians over the observed cochlear length ( & lt ; 1 , 000 microm ) , and instantaneous waveforms show sound propagation along the cochlear partition , supporting the existence of the cochlear traveling wave .
	manualset3
233420	1	427853	16	NULL	NULL	0	NULL	2 blind duplicate samples	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For 2 blind duplicate samples of wine containing 75 mg SO2/kg , the relative standard deviation for repeatability ( RSDr , within-laboratory variation ) was 3.9 % .
	manualset3
233435	3	427853	16	NULL	NULL	0	NULL	wine	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	For 2 blind duplicate samples of wine containing 75 mg SO2/kg , the relative standard deviation for repeatability ( RSDr , within-laboratory variation ) was 3.9 % .
	manualset3
233436	4	427853	16	NULL	NULL	NULL	NULL	75 mg SO2/kg	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For 2 blind duplicate samples of wine containing 75 mg SO2/kg , the relative standard deviation for repeatability ( RSDr , within-laboratory variation ) was 3.9 % .
	manualset3
233438	6	427853	16	NULL	NULL	NULL	NULL	relative standard deviation for repeatability ( RSDr	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For 2 blind duplicate samples of wine containing 75 mg SO2/kg , the relative standard deviation for repeatability ( RSDr , within-laboratory variation ) was 3.9 % .
	manualset3
233440	8	427853	16	NULL	NULL	NULL	NULL	 within-laboratory variation	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For 2 blind duplicate samples of wine containing 75 mg SO2/kg , the relative standard deviation for repeatability ( RSDr , within-laboratory variation ) was 3.9 % .
	manualset3
237516	9	427853	16	NULL	NULL	0	NULL	3.9 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For 2 blind duplicate samples of wine containing 75 mg SO2/kg , the relative standard deviation for repeatability ( RSDr , within-laboratory variation ) was 3.9 % .
	manualset3
234088	1	427854	16	NULL	NULL	0	NULL	3-year olds	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	For 3-year olds , both toedrop and toeheight ( speedpeak ) scaled less well to stair height than normal .
	manualset3
234089	2	427854	16	NULL	NULL	0	NULL	toedrop	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For 3-year olds , both toedrop and toeheight ( speedpeak ) scaled less well to stair height than normal .
	manualset3
234091	3	427854	16	NULL	NULL	0	NULL	toeheight	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For 3-year olds , both toedrop and toeheight ( speedpeak ) scaled less well to stair height than normal .
	manualset3
234095	4	427854	16	NULL	NULL	0	NULL	speedpeak	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For 3-year olds , both toedrop and toeheight ( speedpeak ) scaled less well to stair height than normal .
	manualset3
234097	5	427854	16	NULL	NULL	NULL	NULL	stair height	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For 3-year olds , both toedrop and toeheight ( speedpeak ) scaled less well to stair height than normal .
	manualset3
234147	1	427855	16	NULL	NULL	NULL	NULL	33 mares	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For 33 mares with twins , fixation involved one uterine horn in 23 mares and both horns in 10 mares ( significantly different from equality ) .
	manualset3
234152	3	427855	16	NULL	NULL	NULL	NULL	twins	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For 33 mares with twins , fixation involved one uterine horn in 23 mares and both horns in 10 mares ( significantly different from equality ) .
	manualset3
234154	4	427855	16	NULL	NULL	0	NULL	fixation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For 33 mares with twins , fixation involved one uterine horn in 23 mares and both horns in 10 mares ( significantly different from equality ) .
	manualset3
234155	5	427855	16	NULL	NULL	0	NULL	uterine horn	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	For 33 mares with twins , fixation involved one uterine horn in 23 mares and both horns in 10 mares ( significantly different from equality ) .
	manualset3
234156	6	427855	16	NULL	NULL	NULL	NULL	23 mares	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For 33 mares with twins , fixation involved one uterine horn in 23 mares and both horns in 10 mares ( significantly different from equality ) .
	manualset3
234157	7	427855	16	NULL	NULL	NULL	NULL	horns	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For 33 mares with twins , fixation involved one uterine horn in 23 mares and both horns in 10 mares ( significantly different from equality ) .
	manualset3
234158	8	427855	16	NULL	NULL	NULL	NULL	10 mares	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For 33 mares with twins , fixation involved one uterine horn in 23 mares and both horns in 10 mares ( significantly different from equality ) .
	manualset3
234159	9	427855	16	NULL	NULL	NULL	NULL	equality	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For 33 mares with twins , fixation involved one uterine horn in 23 mares and both horns in 10 mares ( significantly different from equality ) .
	manualset3
234160	1	427856	16	NULL	NULL	0	NULL	60 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	For 60 years , dapsone has been used as a both antibacterial and anti-inflammatory agent .
	manualset3
234161	2	427856	16	NULL	NULL	0	NULL	dapsone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	For 60 years , dapsone has been used as a both antibacterial and anti-inflammatory agent .
	manualset3
234162	3	427856	16	NULL	NULL	NULL	NULL	antibacterial agent	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For 60 years , dapsone has been used as a both antibacterial and anti-inflammatory agent .
	manualset3
234163	4	427856	16	NULL	NULL	NULL	NULL	anti-inflammatory agent	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For 60 years , dapsone has been used as a both antibacterial and anti-inflammatory agent .
	manualset3
232633	1	427857	16	NULL	NULL	0	NULL	Acute pulmonary embolism	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Acute pulmonary embolism ) .
	manualset3
234164	1	427858	16	NULL	NULL	NULL	NULL	Reduction	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Reduction of the functional activity of the calcium pump of the sarcoplasmic reticulum of skeletal muscles in response to cold ) .
	manualset3
234165	2	427858	16	NULL	NULL	NULL	NULL	functional activity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Reduction of the functional activity of the calcium pump of the sarcoplasmic reticulum of skeletal muscles in response to cold ) .
	manualset3
234166	3	427858	16	NULL	NULL	0	NULL	calcium pump	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Reduction of the functional activity of the calcium pump of the sarcoplasmic reticulum of skeletal muscles in response to cold ) .
	manualset3
234167	4	427858	16	NULL	NULL	0	NULL	sarcoplasmic reticulum	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	( Reduction of the functional activity of the calcium pump of the sarcoplasmic reticulum of skeletal muscles in response to cold ) .
	manualset3
234168	5	427858	16	NULL	NULL	0	NULL	skeletal muscles	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	( Reduction of the functional activity of the calcium pump of the sarcoplasmic reticulum of skeletal muscles in response to cold ) .
	manualset3
234169	6	427858	16	NULL	NULL	0	NULL	response to cold	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Reduction of the functional activity of the calcium pump of the sarcoplasmic reticulum of skeletal muscles in response to cold ) .
	manualset3
234170	1	427859	16	NULL	NULL	0	NULL	8	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For 8 and 11 , highly resolved 29Si and 119Sn NMR spectra revealed the first two-bond isotope-induced chemical shifts , 2delta10/11B ( 29Si ) and 2delta10/11B ( 119Sn ) respectively , to be reported .
	manualset3
234171	2	427859	16	NULL	NULL	0	NULL	11	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For 8 and 11 , highly resolved 29Si and 119Sn NMR spectra revealed the first two-bond isotope-induced chemical shifts , 2delta10/11B ( 29Si ) and 2delta10/11B ( 119Sn ) respectively , to be reported .
	manualset3
234172	3	427859	16	NULL	NULL	NULL	NULL	29Si	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For 8 and 11 , highly resolved 29Si and 119Sn NMR spectra revealed the first two-bond isotope-induced chemical shifts , 2delta10/11B ( 29Si ) and 2delta10/11B ( 119Sn ) respectively , to be reported .
	manualset3
234174	4	427859	16	NULL	NULL	NULL	NULL	119Sn	Atom												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For 8 and 11 , highly resolved 29Si and 119Sn NMR spectra revealed the first two-bond isotope-induced chemical shifts , 2delta10/11B ( 29Si ) and 2delta10/11B ( 119Sn ) respectively , to be reported .
	manualset3
234175	5	427859	16	NULL	NULL	NULL	NULL	NMR spectra	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For 8 and 11 , highly resolved 29Si and 119Sn NMR spectra revealed the first two-bond isotope-induced chemical shifts , 2delta10/11B ( 29Si ) and 2delta10/11B ( 119Sn ) respectively , to be reported .
	manualset3
234209	6	427859	16	NULL	NULL	0	NULL	two-bond isotope-induced chemical shifts	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For 8 and 11 , highly resolved 29Si and 119Sn NMR spectra revealed the first two-bond isotope-induced chemical shifts , 2delta10/11B ( 29Si ) and 2delta10/11B ( 119Sn ) respectively , to be reported .
	manualset3
234216	7	427859	16	NULL	NULL	NULL	NULL	2delta10/11B ( 29Si ) 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For 8 and 11 , highly resolved 29Si and 119Sn NMR spectra revealed the first two-bond isotope-induced chemical shifts , 2delta10/11B ( 29Si ) and 2delta10/11B ( 119Sn ) respectively , to be reported .
	manualset3
234221	8	427859	16	NULL	NULL	0	NULL	2delta10/11B ( 119Sn )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For 8 and 11 , highly resolved 29Si and 119Sn NMR spectra revealed the first two-bond isotope-induced chemical shifts , 2delta10/11B ( 29Si ) and 2delta10/11B ( 119Sn ) respectively , to be reported .
	manualset3
234223	2	427860	16	NULL	NULL	NULL	NULL	ALS patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For ALS patients , these values were 21 ( + / -16 ) for statistical method and 55 ( + / -39 ) for multiple point .
	manualset3
234224	3	427860	16	NULL	NULL	0	NULL	21 ( + / -16 )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For ALS patients , these values were 21 ( + / -16 ) for statistical method and 55 ( + / -39 ) for multiple point .
	manualset3
234228	4	427860	16	NULL	NULL	0	NULL	statistical method	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For ALS patients , these values were 21 ( + / -16 ) for statistical method and 55 ( + / -39 ) for multiple point .
	manualset3
234230	5	427860	16	NULL	NULL	0	NULL	55 ( + / -39 )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For ALS patients , these values were 21 ( + / -16 ) for statistical method and 55 ( + / -39 ) for multiple point .
	manualset3
234233	6	427860	16	NULL	NULL	0	NULL	multiple point	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For ALS patients , these values were 21 ( + / -16 ) for statistical method and 55 ( + / -39 ) for multiple point .
	manualset3
236619	1	427861	16	NULL	NULL	0	NULL	BW	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For BW , LRFI boars had a lighter mature BW ( 279 vs. 317 kg ) , an earlier inflection point ( 184 vs. 198 d ) , and a decreased decay parameter ( 127 vs. 134 d ) compared with CTRL boars .
	manualset3
236620	2	427861	16	NULL	NULL	0	NULL	LRFI boars	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For BW , LRFI boars had a lighter mature BW ( 279 vs. 317 kg ) , an earlier inflection point ( 184 vs. 198 d ) , and a decreased decay parameter ( 127 vs. 134 d ) compared with CTRL boars .
	manualset3
236621	3	427861	16	NULL	NULL	0	NULL	BW ( 279 vs. 317 kg )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For BW , LRFI boars had a lighter mature BW ( 279 vs. 317 kg ) , an earlier inflection point ( 184 vs. 198 d ) , and a decreased decay parameter ( 127 vs. 134 d ) compared with CTRL boars .
	manualset3
236622	4	427861	16	NULL	NULL	0	NULL	 inflection point ( 184 vs. 198 d )	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	For BW , LRFI boars had a lighter mature BW ( 279 vs. 317 kg ) , an earlier inflection point ( 184 vs. 198 d ) , and a decreased decay parameter ( 127 vs. 134 d ) compared with CTRL boars .
	manualset3
236623	5	427861	16	NULL	NULL	0	NULL	decay parameter ( 127 vs. 134 d )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For BW , LRFI boars had a lighter mature BW ( 279 vs. 317 kg ) , an earlier inflection point ( 184 vs. 198 d ) , and a decreased decay parameter ( 127 vs. 134 d ) compared with CTRL boars .
	manualset3
236624	6	427861	16	NULL	NULL	0	NULL	CTRL boars	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For BW , LRFI boars had a lighter mature BW ( 279 vs. 317 kg ) , an earlier inflection point ( 184 vs. 198 d ) , and a decreased decay parameter ( 127 vs. 134 d ) compared with CTRL boars .
	manualset3
234240	1	427862	16	NULL	NULL	NULL	NULL	CA 125	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For CA 125 and CA 15.3 , no significant difference in the distribution of marker levels according to histopathological variables was found .
	manualset3
234241	2	427862	16	NULL	NULL	NULL	NULL	CA 15.3	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For CA 125 and CA 15.3 , no significant difference in the distribution of marker levels according to histopathological variables was found .
	manualset3
234243	3	427862	16	NULL	NULL	0	NULL	distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For CA 125 and CA 15.3 , no significant difference in the distribution of marker levels according to histopathological variables was found .
	manualset3
234244	4	427862	16	NULL	NULL	0	NULL	marker levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For CA 125 and CA 15.3 , no significant difference in the distribution of marker levels according to histopathological variables was found .
	manualset3
234246	5	427862	16	NULL	NULL	NULL	NULL	histopathological variables	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For CA 125 and CA 15.3 , no significant difference in the distribution of marker levels according to histopathological variables was found .
	manualset3
237981	6	427862	16	NULL	NULL	0	NULL	difference	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	For CA 125 and CA 15.3 , no significant difference in the distribution of marker levels according to histopathological variables was found .
	manualset3
234254	1	427863	16	NULL	NULL	NULL	NULL	CHD	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For CHD and Pro , we present an explanation of the biexponential decay recently reported by Sension and coworkers ( Tang et al. , J. Phys .
	manualset3
234259	2	427863	16	NULL	NULL	NULL	NULL	Pro	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For CHD and Pro , we present an explanation of the biexponential decay recently reported by Sension and coworkers ( Tang et al. , J. Phys .
	manualset3
234277	3	427863	16	NULL	NULL	NULL	NULL	explanation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For CHD and Pro , we present an explanation of the biexponential decay recently reported by Sension and coworkers ( Tang et al. , J. Phys .
	manualset3
234280	4	427863	16	NULL	NULL	NULL	NULL	biexponential decay	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For CHD and Pro , we present an explanation of the biexponential decay recently reported by Sension and coworkers ( Tang et al. , J. Phys .
	manualset3
234281	5	427863	16	NULL	NULL	NULL	NULL	Sension and coworkers	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For CHD and Pro , we present an explanation of the biexponential decay recently reported by Sension and coworkers ( Tang et al. , J. Phys .
	manualset3
234285	6	427863	16	NULL	NULL	NULL	NULL	Tang et al. , J. Phys	Citation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For CHD and Pro , we present an explanation of the biexponential decay recently reported by Sension and coworkers ( Tang et al. , J. Phys .
	manualset3
234396	1	427864	16	NULL	NULL	0	NULL	CIN2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For CIN2 , the sensitivity and specificity for diffuse staining were 81.1 % and 95.4 % , respectively .
	manualset3
234397	2	427864	16	NULL	NULL	0	NULL	diffuse staining	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For CIN2 , the sensitivity and specificity for diffuse staining were 81.1 % and 95.4 % , respectively .
	manualset3
234398	3	427864	16	NULL	NULL	0	NULL	81.1 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For CIN2 , the sensitivity and specificity for diffuse staining were 81.1 % and 95.4 % , respectively .
	manualset3
234399	4	427864	16	NULL	NULL	0	NULL	95.4 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For CIN2 , the sensitivity and specificity for diffuse staining were 81.1 % and 95.4 % , respectively .
	manualset3
237982	5	427864	16	NULL	NULL	0	NULL	sensitivity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For CIN2 , the sensitivity and specificity for diffuse staining were 81.1 % and 95.4 % , respectively .
	manualset3
237983	6	427864	16	NULL	NULL	0	NULL	specificity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For CIN2 , the sensitivity and specificity for diffuse staining were 81.1 % and 95.4 % , respectively .
	manualset3
234417	1	427865	16	NULL	NULL	0	NULL	CY	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For CY , MISO was a better sensitizer than METRO at RT and 37 degrees C , but the magnitude of the chemosensitization by MISO and METRO became identical at 41.5 degrees C. Notably , the chemosensitization was substantially enhanced at 41.5 degrees C , whereas neither 41.5 degrees C-heat , NIs or combined NI and heat prolonged the TG time .
	manualset3
234418	2	427865	16	NULL	NULL	0	NULL	MISO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For CY , MISO was a better sensitizer than METRO at RT and 37 degrees C , but the magnitude of the chemosensitization by MISO and METRO became identical at 41.5 degrees C. Notably , the chemosensitization was substantially enhanced at 41.5 degrees C , whereas neither 41.5 degrees C-heat , NIs or combined NI and heat prolonged the TG time .
	manualset3
234430	3	427865	16	NULL	NULL	0	NULL	sensitizer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For CY , MISO was a better sensitizer than METRO at RT and 37 degrees C , but the magnitude of the chemosensitization by MISO and METRO became identical at 41.5 degrees C. Notably , the chemosensitization was substantially enhanced at 41.5 degrees C , whereas neither 41.5 degrees C-heat , NIs or combined NI and heat prolonged the TG time .
	manualset3
234431	4	427865	16	NULL	NULL	0	NULL	METRO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For CY , MISO was a better sensitizer than METRO at RT and 37 degrees C , but the magnitude of the chemosensitization by MISO and METRO became identical at 41.5 degrees C. Notably , the chemosensitization was substantially enhanced at 41.5 degrees C , whereas neither 41.5 degrees C-heat , NIs or combined NI and heat prolonged the TG time .
	manualset3
234436	5	427865	16	NULL	NULL	NULL	NULL	 RT and 37 degrees C	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For CY , MISO was a better sensitizer than METRO at RT and 37 degrees C , but the magnitude of the chemosensitization by MISO and METRO became identical at 41.5 degrees C. Notably , the chemosensitization was substantially enhanced at 41.5 degrees C , whereas neither 41.5 degrees C-heat , NIs or combined NI and heat prolonged the TG time .
	manualset3
234441	7	427865	16	NULL	NULL	0	NULL	magnitude	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For CY , MISO was a better sensitizer than METRO at RT and 37 degrees C , but the magnitude of the chemosensitization by MISO and METRO became identical at 41.5 degrees C. Notably , the chemosensitization was substantially enhanced at 41.5 degrees C , whereas neither 41.5 degrees C-heat , NIs or combined NI and heat prolonged the TG time .
	manualset3
234444	8	427865	16	NULL	NULL	0	NULL	chemosensitization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For CY , MISO was a better sensitizer than METRO at RT and 37 degrees C , but the magnitude of the chemosensitization by MISO and METRO became identical at 41.5 degrees C. Notably , the chemosensitization was substantially enhanced at 41.5 degrees C , whereas neither 41.5 degrees C-heat , NIs or combined NI and heat prolonged the TG time .
	manualset3
234445	9	427865	16	NULL	NULL	0	NULL	MISO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For CY , MISO was a better sensitizer than METRO at RT and 37 degrees C , but the magnitude of the chemosensitization by MISO and METRO became identical at 41.5 degrees C. Notably , the chemosensitization was substantially enhanced at 41.5 degrees C , whereas neither 41.5 degrees C-heat , NIs or combined NI and heat prolonged the TG time .
	manualset3
234446	10	427865	16	NULL	NULL	0	NULL	METRO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For CY , MISO was a better sensitizer than METRO at RT and 37 degrees C , but the magnitude of the chemosensitization by MISO and METRO became identical at 41.5 degrees C. Notably , the chemosensitization was substantially enhanced at 41.5 degrees C , whereas neither 41.5 degrees C-heat , NIs or combined NI and heat prolonged the TG time .
	manualset3
234450	11	427865	16	NULL	NULL	0	NULL	41.5 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For CY , MISO was a better sensitizer than METRO at RT and 37 degrees C , but the magnitude of the chemosensitization by MISO and METRO became identical at 41.5 degrees C. Notably , the chemosensitization was substantially enhanced at 41.5 degrees C , whereas neither 41.5 degrees C-heat , NIs or combined NI and heat prolonged the TG time .
	manualset3
234452	12	427865	16	NULL	NULL	0	NULL	chemosensitization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For CY , MISO was a better sensitizer than METRO at RT and 37 degrees C , but the magnitude of the chemosensitization by MISO and METRO became identical at 41.5 degrees C. Notably , the chemosensitization was substantially enhanced at 41.5 degrees C , whereas neither 41.5 degrees C-heat , NIs or combined NI and heat prolonged the TG time .
	manualset3
234453	13	427865	16	NULL	NULL	0	NULL	41.5 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For CY , MISO was a better sensitizer than METRO at RT and 37 degrees C , but the magnitude of the chemosensitization by MISO and METRO became identical at 41.5 degrees C. Notably , the chemosensitization was substantially enhanced at 41.5 degrees C , whereas neither 41.5 degrees C-heat , NIs or combined NI and heat prolonged the TG time .
	manualset3
234454	14	427865	16	NULL	NULL	0	NULL	41.5 degrees C	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For CY , MISO was a better sensitizer than METRO at RT and 37 degrees C , but the magnitude of the chemosensitization by MISO and METRO became identical at 41.5 degrees C. Notably , the chemosensitization was substantially enhanced at 41.5 degrees C , whereas neither 41.5 degrees C-heat , NIs or combined NI and heat prolonged the TG time .
	manualset3
234455	15	427865	16	NULL	NULL	0	NULL	heat	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	For CY , MISO was a better sensitizer than METRO at RT and 37 degrees C , but the magnitude of the chemosensitization by MISO and METRO became identical at 41.5 degrees C. Notably , the chemosensitization was substantially enhanced at 41.5 degrees C , whereas neither 41.5 degrees C-heat , NIs or combined NI and heat prolonged the TG time .
	manualset3
234456	16	427865	16	NULL	NULL	NULL	NULL	NIs	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For CY , MISO was a better sensitizer than METRO at RT and 37 degrees C , but the magnitude of the chemosensitization by MISO and METRO became identical at 41.5 degrees C. Notably , the chemosensitization was substantially enhanced at 41.5 degrees C , whereas neither 41.5 degrees C-heat , NIs or combined NI and heat prolonged the TG time .
	manualset3
234457	17	427865	16	NULL	NULL	NULL	NULL	NI	LaboratoryExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For CY , MISO was a better sensitizer than METRO at RT and 37 degrees C , but the magnitude of the chemosensitization by MISO and METRO became identical at 41.5 degrees C. Notably , the chemosensitization was substantially enhanced at 41.5 degrees C , whereas neither 41.5 degrees C-heat , NIs or combined NI and heat prolonged the TG time .
	manualset3
234459	18	427865	16	NULL	NULL	0	NULL	heat	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	For CY , MISO was a better sensitizer than METRO at RT and 37 degrees C , but the magnitude of the chemosensitization by MISO and METRO became identical at 41.5 degrees C. Notably , the chemosensitization was substantially enhanced at 41.5 degrees C , whereas neither 41.5 degrees C-heat , NIs or combined NI and heat prolonged the TG time .
	manualset3
234469	19	427865	16	NULL	NULL	NULL	NULL	TG time	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For CY , MISO was a better sensitizer than METRO at RT and 37 degrees C , but the magnitude of the chemosensitization by MISO and METRO became identical at 41.5 degrees C. Notably , the chemosensitization was substantially enhanced at 41.5 degrees C , whereas neither 41.5 degrees C-heat , NIs or combined NI and heat prolonged the TG time .
	manualset3
236600	1	427866	16	NULL	NULL	0	NULL	FM	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For FM of the 1-kHz carrier , performance improved markedly with increasing TSS , especially for the lower FM rates ; there was no change in performance with TSS for the 20-Hz modulation rate .
	manualset3
236601	2	427866	16	NULL	NULL	NULL	NULL	1-kHz carrier	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For FM of the 1-kHz carrier , performance improved markedly with increasing TSS , especially for the lower FM rates ; there was no change in performance with TSS for the 20-Hz modulation rate .
	manualset3
236602	3	427866	16	NULL	NULL	0	NULL	performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For FM of the 1-kHz carrier , performance improved markedly with increasing TSS , especially for the lower FM rates ; there was no change in performance with TSS for the 20-Hz modulation rate .
	manualset3
236603	4	427866	16	NULL	NULL	NULL	NULL	TSS	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For FM of the 1-kHz carrier , performance improved markedly with increasing TSS , especially for the lower FM rates ; there was no change in performance with TSS for the 20-Hz modulation rate .
	manualset3
236604	5	427866	16	NULL	NULL	0	NULL	FM rates	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For FM of the 1-kHz carrier , performance improved markedly with increasing TSS , especially for the lower FM rates ; there was no change in performance with TSS for the 20-Hz modulation rate .
	manualset3
236605	6	427866	16	NULL	NULL	0	NULL	performance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For FM of the 1-kHz carrier , performance improved markedly with increasing TSS , especially for the lower FM rates ; there was no change in performance with TSS for the 20-Hz modulation rate .
	manualset3
236606	7	427866	16	NULL	NULL	NULL	NULL	TSS	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For FM of the 1-kHz carrier , performance improved markedly with increasing TSS , especially for the lower FM rates ; there was no change in performance with TSS for the 20-Hz modulation rate .
	manualset3
236607	8	427866	16	NULL	NULL	0	NULL	20-Hz modulation rate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For FM of the 1-kHz carrier , performance improved markedly with increasing TSS , especially for the lower FM rates ; there was no change in performance with TSS for the 20-Hz modulation rate .
	manualset3
237984	9	427866	16	NULL	NULL	0	NULL	change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For FM of the 1-kHz carrier , performance improved markedly with increasing TSS , especially for the lower FM rates ; there was no change in performance with TSS for the 20-Hz modulation rate .
	manualset3
234538	1	427867	16	NULL	NULL	0	NULL	FMDV	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For FMDV , as in other picornaviruses , viral infection is dependent on the correct function of the IRES ; therefore , the IRES region itself constitutes a useful target of antiviral drugs .
	manualset3
234539	2	427867	16	NULL	NULL	0	NULL	picornaviruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For FMDV , as in other picornaviruses , viral infection is dependent on the correct function of the IRES ; therefore , the IRES region itself constitutes a useful target of antiviral drugs .
	manualset3
234540	3	427867	16	NULL	NULL	0	NULL	viral infection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For FMDV , as in other picornaviruses , viral infection is dependent on the correct function of the IRES ; therefore , the IRES region itself constitutes a useful target of antiviral drugs .
	manualset3
234542	4	427867	16	NULL	NULL	NULL	NULL	function	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For FMDV , as in other picornaviruses , viral infection is dependent on the correct function of the IRES ; therefore , the IRES region itself constitutes a useful target of antiviral drugs .
	manualset3
234547	5	427867	16	NULL	NULL	0	NULL	IRES	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	For FMDV , as in other picornaviruses , viral infection is dependent on the correct function of the IRES ; therefore , the IRES region itself constitutes a useful target of antiviral drugs .
	manualset3
234548	6	427867	16	NULL	NULL	NULL	NULL	IRES region	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For FMDV , as in other picornaviruses , viral infection is dependent on the correct function of the IRES ; therefore , the IRES region itself constitutes a useful target of antiviral drugs .
	manualset3
237957	7	427867	16	NULL	NULL	0	NULL	antiviral drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	For FMDV , as in other picornaviruses , viral infection is dependent on the correct function of the IRES ; therefore , the IRES region itself constitutes a useful target of antiviral drugs .
	manualset3
237985	8	427867	16	NULL	NULL	0	NULL	target	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	For FMDV , as in other picornaviruses , viral infection is dependent on the correct function of the IRES ; therefore , the IRES region itself constitutes a useful target of antiviral drugs .
	manualset3
234549	1	427868	16	NULL	NULL	NULL	NULL	Reduction	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Reduction of traumatic dislocation of the shoulder .
	manualset3
234550	2	427868	16	NULL	NULL	0	NULL	traumatic dislocation	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Reduction of traumatic dislocation of the shoulder .
	manualset3
234551	3	427868	16	NULL	NULL	0	NULL	shoulder	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Reduction of traumatic dislocation of the shoulder .
	manualset3
234622	1	427869	16	NULL	NULL	0	NULL	H. placei	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For H. placei the reductions were 98 % ( 85-99 .7 % ) for MXD , 0.7 % ( -226 to 70 % ) for IVM and 100 % for LEV .
	manualset3
234623	2	427869	16	NULL	NULL	NULL	NULL	reductions	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For H. placei the reductions were 98 % ( 85-99 .7 % ) for MXD , 0.7 % ( -226 to 70 % ) for IVM and 100 % for LEV .
	manualset3
234624	3	427869	16	NULL	NULL	NULL	NULL	98 % ( 85-99 .7 % )	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For H. placei the reductions were 98 % ( 85-99 .7 % ) for MXD , 0.7 % ( -226 to 70 % ) for IVM and 100 % for LEV .
	manualset3
234625	4	427869	16	NULL	NULL	NULL	NULL	MXD	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For H. placei the reductions were 98 % ( 85-99 .7 % ) for MXD , 0.7 % ( -226 to 70 % ) for IVM and 100 % for LEV .
	manualset3
234626	5	427869	16	NULL	NULL	NULL	NULL	0.7 % ( -226 to 70 % )	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For H. placei the reductions were 98 % ( 85-99 .7 % ) for MXD , 0.7 % ( -226 to 70 % ) for IVM and 100 % for LEV .
	manualset3
234627	6	427869	16	NULL	NULL	NULL	NULL	IVM	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For H. placei the reductions were 98 % ( 85-99 .7 % ) for MXD , 0.7 % ( -226 to 70 % ) for IVM and 100 % for LEV .
	manualset3
234628	7	427869	16	NULL	NULL	NULL	NULL	100 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For H. placei the reductions were 98 % ( 85-99 .7 % ) for MXD , 0.7 % ( -226 to 70 % ) for IVM and 100 % for LEV .
	manualset3
237956	8	427869	16	NULL	NULL	0	NULL	LEV	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	For H. placei the reductions were 98 % ( 85-99 .7 % ) for MXD , 0.7 % ( -226 to 70 % ) for IVM and 100 % for LEV .
	manualset3
234629	1	427870	16	NULL	NULL	0	NULL	PAX7	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For PAX7 and PAX7-FKHR , there was a consistent pattern of co-expression of the 4 isoforms in RMS tumors : Q+GL - ) Q+GL + ) / = Q-GL - ) Q-GL + .
	manualset3
234630	2	427870	16	NULL	NULL	0	NULL	PAX7-FKHR	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For PAX7 and PAX7-FKHR , there was a consistent pattern of co-expression of the 4 isoforms in RMS tumors : Q+GL - ) Q+GL + ) / = Q-GL - ) Q-GL + .
	manualset3
234631	3	427870	16	NULL	NULL	NULL	NULL	pattern of co-expression	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For PAX7 and PAX7-FKHR , there was a consistent pattern of co-expression of the 4 isoforms in RMS tumors : Q+GL - ) Q+GL + ) / = Q-GL - ) Q-GL + .
	manualset3
234632	4	427870	16	NULL	NULL	NULL	NULL	4 isoforms	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For PAX7 and PAX7-FKHR , there was a consistent pattern of co-expression of the 4 isoforms in RMS tumors : Q+GL - ) Q+GL + ) / = Q-GL - ) Q-GL + .
	manualset3
234634	6	427870	16	NULL	NULL	0	NULL	RMS tumors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For PAX7 and PAX7-FKHR , there was a consistent pattern of co-expression of the 4 isoforms in RMS tumors : Q+GL - ) Q+GL + ) / = Q-GL - ) Q-GL + .
	manualset3
234635	7	427870	16	NULL	NULL	0	NULL	 Q+GL - ) Q+GL + ) / = Q-GL - ) Q-GL + .	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For PAX7 and PAX7-FKHR , there was a consistent pattern of co-expression of the 4 isoforms in RMS tumors : Q+GL - ) Q+GL + ) / = Q-GL - ) Q-GL + .
	manualset3
234636	1	427871	16	NULL	NULL	0	NULL	TBC	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For TBC ) 85 ng/ml , no patient developed grade II-IV aGVHD , 10 developed mild aGVHD and 30 had no aGVHD .
	manualset3
234637	2	427871	16	NULL	NULL	NULL	NULL	85 ng/ml	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For TBC ) 85 ng/ml , no patient developed grade II-IV aGVHD , 10 developed mild aGVHD and 30 had no aGVHD .
	manualset3
234640	3	427871	16	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	For TBC ) 85 ng/ml , no patient developed grade II-IV aGVHD , 10 developed mild aGVHD and 30 had no aGVHD .
	manualset3
234641	4	427871	16	NULL	NULL	0	NULL	grade II-IV aGVHD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	For TBC ) 85 ng/ml , no patient developed grade II-IV aGVHD , 10 developed mild aGVHD and 30 had no aGVHD .
	manualset3
234642	5	427871	16	NULL	NULL	0	NULL	10	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For TBC ) 85 ng/ml , no patient developed grade II-IV aGVHD , 10 developed mild aGVHD and 30 had no aGVHD .
	manualset3
234643	6	427871	16	NULL	NULL	0	NULL	mild aGVHD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	For TBC ) 85 ng/ml , no patient developed grade II-IV aGVHD , 10 developed mild aGVHD and 30 had no aGVHD .
	manualset3
234644	7	427871	16	NULL	NULL	0	NULL	30	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For TBC ) 85 ng/ml , no patient developed grade II-IV aGVHD , 10 developed mild aGVHD and 30 had no aGVHD .
	manualset3
234645	8	427871	16	NULL	NULL	0	NULL	aGVHD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	For TBC ) 85 ng/ml , no patient developed grade II-IV aGVHD , 10 developed mild aGVHD and 30 had no aGVHD .
	manualset3
236608	1	427872	16	NULL	NULL	NULL	NULL	database	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For a diverse database of RNA sequences , base pairs in the predicted minimum free energy structure that are predicted by the partition function to have high base pairing probability have a significantly higher positive predictive value for known base pairs .
	manualset3
236609	2	427872	16	NULL	NULL	0	NULL	RNA sequences	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	For a diverse database of RNA sequences , base pairs in the predicted minimum free energy structure that are predicted by the partition function to have high base pairing probability have a significantly higher positive predictive value for known base pairs .
	manualset3
236610	3	427872	16	NULL	NULL	NULL	NULL	base pairs	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For a diverse database of RNA sequences , base pairs in the predicted minimum free energy structure that are predicted by the partition function to have high base pairing probability have a significantly higher positive predictive value for known base pairs .
	manualset3
237510	4	427872	16	NULL	NULL	0	NULL	free energy structure	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For a diverse database of RNA sequences , base pairs in the predicted minimum free energy structure that are predicted by the partition function to have high base pairing probability have a significantly higher positive predictive value for known base pairs .
	manualset3
237511	5	427872	16	NULL	NULL	0	NULL	partition function	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For a diverse database of RNA sequences , base pairs in the predicted minimum free energy structure that are predicted by the partition function to have high base pairing probability have a significantly higher positive predictive value for known base pairs .
	manualset3
237512	6	427872	16	NULL	NULL	0	NULL	 base pairing probability	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For a diverse database of RNA sequences , base pairs in the predicted minimum free energy structure that are predicted by the partition function to have high base pairing probability have a significantly higher positive predictive value for known base pairs .
	manualset3
237513	7	427872	16	NULL	NULL	0	NULL	predictive value	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For a diverse database of RNA sequences , base pairs in the predicted minimum free energy structure that are predicted by the partition function to have high base pairing probability have a significantly higher positive predictive value for known base pairs .
	manualset3
237514	8	427872	16	NULL	NULL	0	NULL	base pairs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	For a diverse database of RNA sequences , base pairs in the predicted minimum free energy structure that are predicted by the partition function to have high base pairing probability have a significantly higher positive predictive value for known base pairs .
	manualset3
237958	1	427873	16	NULL	NULL	0	NULL	 fifth isolate of S. parauberis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For a fifth isolate of S. parauberis , six 16S rRNA genes were indicated by the universal probe but only five when hybridised to the species-specific probe , indicating sequence variation ( microheterogeneity ) within the probe target region .
	manualset3
237959	2	427873	16	NULL	NULL	0	NULL	six 16S rRNA genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	For a fifth isolate of S. parauberis , six 16S rRNA genes were indicated by the universal probe but only five when hybridised to the species-specific probe , indicating sequence variation ( microheterogeneity ) within the probe target region .
	manualset3
237960	3	427873	16	NULL	NULL	0	NULL	universal probe	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	For a fifth isolate of S. parauberis , six 16S rRNA genes were indicated by the universal probe but only five when hybridised to the species-specific probe , indicating sequence variation ( microheterogeneity ) within the probe target region .
	manualset3
237961	4	427873	16	NULL	NULL	0	NULL	five	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For a fifth isolate of S. parauberis , six 16S rRNA genes were indicated by the universal probe but only five when hybridised to the species-specific probe , indicating sequence variation ( microheterogeneity ) within the probe target region .
	manualset3
237962	5	427873	16	NULL	NULL	0	NULL	species-specific probe	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	For a fifth isolate of S. parauberis , six 16S rRNA genes were indicated by the universal probe but only five when hybridised to the species-specific probe , indicating sequence variation ( microheterogeneity ) within the probe target region .
	manualset3
237963	6	427873	16	NULL	NULL	0	NULL	sequence variation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For a fifth isolate of S. parauberis , six 16S rRNA genes were indicated by the universal probe but only five when hybridised to the species-specific probe , indicating sequence variation ( microheterogeneity ) within the probe target region .
	manualset3
237964	7	427873	16	NULL	NULL	0	NULL	microheterogeneity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For a fifth isolate of S. parauberis , six 16S rRNA genes were indicated by the universal probe but only five when hybridised to the species-specific probe , indicating sequence variation ( microheterogeneity ) within the probe target region .
	manualset3
237965	8	427873	16	NULL	NULL	0	NULL	probe target region	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	For a fifth isolate of S. parauberis , six 16S rRNA genes were indicated by the universal probe but only five when hybridised to the species-specific probe , indicating sequence variation ( microheterogeneity ) within the probe target region .
	manualset3
237966	1	427874	16	NULL	NULL	0	NULL	two-dimensional sheet of tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	For a two-dimensional sheet of tissue , the intracellular and extracellular conductivity tensors can be visualized as two ellipses .
	manualset3
237967	2	427874	16	NULL	NULL	0	NULL	intracellular conductivity tensors	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For a two-dimensional sheet of tissue , the intracellular and extracellular conductivity tensors can be visualized as two ellipses .
	manualset3
237968	3	427874	16	NULL	NULL	0	NULL	extracellular conductivity tensors	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For a two-dimensional sheet of tissue , the intracellular and extracellular conductivity tensors can be visualized as two ellipses .
	manualset3
237969	4	427874	16	NULL	NULL	0	NULL	two ellipses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For a two-dimensional sheet of tissue , the intracellular and extracellular conductivity tensors can be visualized as two ellipses .
	manualset3
237970	1	427875	16	NULL	NULL	NULL	NULL	typical case	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For a typical case reflecting United States teleworker patterns , the analysis found that telework has the potential to reduce air emissions .
	manualset3
237971	2	427875	16	NULL	NULL	0	NULL	United States teleworker patterns	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For a typical case reflecting United States teleworker patterns , the analysis found that telework has the potential to reduce air emissions .
	manualset3
237972	3	427875	16	NULL	NULL	0	NULL	analysis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For a typical case reflecting United States teleworker patterns , the analysis found that telework has the potential to reduce air emissions .
	manualset3
237973	4	427875	16	NULL	NULL	0	NULL	telework	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For a typical case reflecting United States teleworker patterns , the analysis found that telework has the potential to reduce air emissions .
	manualset3
237974	5	427875	16	NULL	NULL	0	NULL	potential	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For a typical case reflecting United States teleworker patterns , the analysis found that telework has the potential to reduce air emissions .
	manualset3
237975	6	427875	16	NULL	NULL	0	NULL	air emissions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For a typical case reflecting United States teleworker patterns , the analysis found that telework has the potential to reduce air emissions .
	manualset3
237976	1	427876	16	NULL	NULL	0	NULL	20 years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	For about 20 years , it was generally accepted that the amphipathic helices of apoA-I lie parallel to the acyl chains of the phospholipids ( `` picket fence '' model ) .
	manualset3
237977	2	427876	16	NULL	NULL	0	NULL	 amphipathic helices of apoA-I	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	For about 20 years , it was generally accepted that the amphipathic helices of apoA-I lie parallel to the acyl chains of the phospholipids ( `` picket fence '' model ) .
	manualset3
237978	3	427876	16	NULL	NULL	0	NULL	acyl chains of the phospholipids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For about 20 years , it was generally accepted that the amphipathic helices of apoA-I lie parallel to the acyl chains of the phospholipids ( `` picket fence '' model ) .
	manualset3
237979	4	427876	16	NULL	NULL	NULL	NULL	picket fence '' model	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For about 20 years , it was generally accepted that the amphipathic helices of apoA-I lie parallel to the acyl chains of the phospholipids ( `` picket fence '' model ) .
	manualset3
237980	1	427877	16	NULL	NULL	0	NULL	agency personnel	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	For agency personnel working with the topic of patient safety , that change has created a need to develop greater awareness of the current patient safety initiatives underway at leading health care systems in order to determine where AHRQ might best play a role in helping these systems more rapidly adopt new practices to improve patient safety .
	manualset3
237986	2	427877	16	NULL	NULL	0	NULL	patient safety	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For agency personnel working with the topic of patient safety , that change has created a need to develop greater awareness of the current patient safety initiatives underway at leading health care systems in order to determine where AHRQ might best play a role in helping these systems more rapidly adopt new practices to improve patient safety .
	manualset3
237987	3	427877	16	NULL	NULL	0	NULL	change	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For agency personnel working with the topic of patient safety , that change has created a need to develop greater awareness of the current patient safety initiatives underway at leading health care systems in order to determine where AHRQ might best play a role in helping these systems more rapidly adopt new practices to improve patient safety .
	manualset3
237988	4	427877	16	NULL	NULL	NULL	NULL	patient safety initiatives	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For agency personnel working with the topic of patient safety , that change has created a need to develop greater awareness of the current patient safety initiatives underway at leading health care systems in order to determine where AHRQ might best play a role in helping these systems more rapidly adopt new practices to improve patient safety .
	manualset3
238017	5	427877	16	NULL	NULL	0	NULL	health care systems	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	For agency personnel working with the topic of patient safety , that change has created a need to develop greater awareness of the current patient safety initiatives underway at leading health care systems in order to determine where AHRQ might best play a role in helping these systems more rapidly adopt new practices to improve patient safety .
	manualset3
238018	6	427877	16	NULL	NULL	NULL	NULL	AHRQ	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For agency personnel working with the topic of patient safety , that change has created a need to develop greater awareness of the current patient safety initiatives underway at leading health care systems in order to determine where AHRQ might best play a role in helping these systems more rapidly adopt new practices to improve patient safety .
	manualset3
238019	7	427877	16	NULL	NULL	0	NULL	practices	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For agency personnel working with the topic of patient safety , that change has created a need to develop greater awareness of the current patient safety initiatives underway at leading health care systems in order to determine where AHRQ might best play a role in helping these systems more rapidly adopt new practices to improve patient safety .
	manualset3
238020	8	427877	16	NULL	NULL	0	NULL	patient safety	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For agency personnel working with the topic of patient safety , that change has created a need to develop greater awareness of the current patient safety initiatives underway at leading health care systems in order to determine where AHRQ might best play a role in helping these systems more rapidly adopt new practices to improve patient safety .
	manualset3
239607	9	427877	16	NULL	NULL	0	NULL	topic	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For agency personnel working with the topic of patient safety , that change has created a need to develop greater awareness of the current patient safety initiatives underway at leading health care systems in order to determine where AHRQ might best play a role in helping these systems more rapidly adopt new practices to improve patient safety .
	manualset3
239608	10	427877	16	NULL	NULL	0	NULL	need	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For agency personnel working with the topic of patient safety , that change has created a need to develop greater awareness of the current patient safety initiatives underway at leading health care systems in order to determine where AHRQ might best play a role in helping these systems more rapidly adopt new practices to improve patient safety .
	manualset3
239609	10	427877	16	NULL	NULL	NULL	NULL	awareness	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For agency personnel working with the topic of patient safety , that change has created a need to develop greater awareness of the current patient safety initiatives underway at leading health care systems in order to determine where AHRQ might best play a role in helping these systems more rapidly adopt new practices to improve patient safety .
	manualset3
239618	11	427877	16	NULL	NULL	0	NULL	systems	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	For agency personnel working with the topic of patient safety , that change has created a need to develop greater awareness of the current patient safety initiatives underway at leading health care systems in order to determine where AHRQ might best play a role in helping these systems more rapidly adopt new practices to improve patient safety .
	manualset3
238021	1	427878	16	NULL	NULL	0	NULL	S. pneumoniae isolates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For all S. pneumoniae isolates tested , gemifloxacin MICs were & lt ; / = 0.5 microgram/ml , suggesting that gemifloxacin has the potential to be used as a treatment for pneumococcal infections , including those arising from isolates resistant to beta-lactams and macrolides .
	manualset3
238022	2	427878	16	NULL	NULL	0	NULL	gemifloxacin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	For all S. pneumoniae isolates tested , gemifloxacin MICs were & lt ; / = 0.5 microgram/ml , suggesting that gemifloxacin has the potential to be used as a treatment for pneumococcal infections , including those arising from isolates resistant to beta-lactams and macrolides .
	manualset3
238023	3	427878	16	NULL	NULL	0	NULL	MICs	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For all S. pneumoniae isolates tested , gemifloxacin MICs were & lt ; / = 0.5 microgram/ml , suggesting that gemifloxacin has the potential to be used as a treatment for pneumococcal infections , including those arising from isolates resistant to beta-lactams and macrolides .
	manualset3
238024	4	427878	16	NULL	NULL	0	NULL	0.5 microgram/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For all S. pneumoniae isolates tested , gemifloxacin MICs were & lt ; / = 0.5 microgram/ml , suggesting that gemifloxacin has the potential to be used as a treatment for pneumococcal infections , including those arising from isolates resistant to beta-lactams and macrolides .
	manualset3
238025	5	427878	16	NULL	NULL	0	NULL	gemifloxacin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	For all S. pneumoniae isolates tested , gemifloxacin MICs were & lt ; / = 0.5 microgram/ml , suggesting that gemifloxacin has the potential to be used as a treatment for pneumococcal infections , including those arising from isolates resistant to beta-lactams and macrolides .
	manualset3
238026	6	427878	16	NULL	NULL	0	NULL	potential	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For all S. pneumoniae isolates tested , gemifloxacin MICs were & lt ; / = 0.5 microgram/ml , suggesting that gemifloxacin has the potential to be used as a treatment for pneumococcal infections , including those arising from isolates resistant to beta-lactams and macrolides .
	manualset3
238027	7	427878	16	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For all S. pneumoniae isolates tested , gemifloxacin MICs were & lt ; / = 0.5 microgram/ml , suggesting that gemifloxacin has the potential to be used as a treatment for pneumococcal infections , including those arising from isolates resistant to beta-lactams and macrolides .
	manualset3
238028	8	427878	16	NULL	NULL	0	NULL	pneumococcal infections	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	For all S. pneumoniae isolates tested , gemifloxacin MICs were & lt ; / = 0.5 microgram/ml , suggesting that gemifloxacin has the potential to be used as a treatment for pneumococcal infections , including those arising from isolates resistant to beta-lactams and macrolides .
	manualset3
238029	9	427878	16	NULL	NULL	0	NULL	isolates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For all S. pneumoniae isolates tested , gemifloxacin MICs were & lt ; / = 0.5 microgram/ml , suggesting that gemifloxacin has the potential to be used as a treatment for pneumococcal infections , including those arising from isolates resistant to beta-lactams and macrolides .
	manualset3
238030	10	427878	16	NULL	NULL	NULL	NULL	beta-lactams	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For all S. pneumoniae isolates tested , gemifloxacin MICs were & lt ; / = 0.5 microgram/ml , suggesting that gemifloxacin has the potential to be used as a treatment for pneumococcal infections , including those arising from isolates resistant to beta-lactams and macrolides .
	manualset3
238031	11	427878	16	NULL	NULL	NULL	NULL	macrolides	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For all S. pneumoniae isolates tested , gemifloxacin MICs were & lt ; / = 0.5 microgram/ml , suggesting that gemifloxacin has the potential to be used as a treatment for pneumococcal infections , including those arising from isolates resistant to beta-lactams and macrolides .
	manualset3
238032	1	427879	16	NULL	NULL	0	NULL	 NRTIs and their combinations	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	For all analyzed NRTIs and their combinations , model-predicted macroscopic parameters ( efficacy , fitness and toxicity ) were consistent with observations .
	manualset3
238033	2	427879	16	NULL	NULL	0	NULL	model-predicted macroscopic parameters	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	For all analyzed NRTIs and their combinations , model-predicted macroscopic parameters ( efficacy , fitness and toxicity ) were consistent with observations .
	manualset3
238034	3	427879	16	NULL	NULL	NULL	NULL	efficacy	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For all analyzed NRTIs and their combinations , model-predicted macroscopic parameters ( efficacy , fitness and toxicity ) were consistent with observations .
	manualset3
238035	4	427879	16	NULL	NULL	NULL	NULL	fitness	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For all analyzed NRTIs and their combinations , model-predicted macroscopic parameters ( efficacy , fitness and toxicity ) were consistent with observations .
	manualset3
238036	5	427879	16	NULL	NULL	NULL	NULL	toxicity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For all analyzed NRTIs and their combinations , model-predicted macroscopic parameters ( efficacy , fitness and toxicity ) were consistent with observations .
	manualset3
238037	6	427879	16	NULL	NULL	0	NULL	observations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For all analyzed NRTIs and their combinations , model-predicted macroscopic parameters ( efficacy , fitness and toxicity ) were consistent with observations .
	manualset3
238038	1	427880	16	NULL	NULL	0	NULL	doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For all doses tested , vHSGFP/P35del caused lower mortality than vHSGFP .
	manualset3
238039	2	427880	16	NULL	NULL	0	NULL	vHSGFP/P35del	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For all doses tested , vHSGFP/P35del caused lower mortality than vHSGFP .
	manualset3
238040	3	427880	16	NULL	NULL	0	NULL	lower mortality	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For all doses tested , vHSGFP/P35del caused lower mortality than vHSGFP .
	manualset3
238041	4	427880	16	NULL	NULL	0	NULL	vHSGFP	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For all doses tested , vHSGFP/P35del caused lower mortality than vHSGFP .
	manualset3
238042	1	427881	16	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	For all patients but 1 , conditioning regimens were based on fludarabine ( Flu ) , which was combined with other chemotherapy drugs in 50 cases ( 74 % ) and with total body irradiation ( TBI ) in 17 ( 25 % ) .
	manualset3
238043	2	427881	16	NULL	NULL	0	NULL	1	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For all patients but 1 , conditioning regimens were based on fludarabine ( Flu ) , which was combined with other chemotherapy drugs in 50 cases ( 74 % ) and with total body irradiation ( TBI ) in 17 ( 25 % ) .
	manualset3
238044	3	427881	16	NULL	NULL	0	NULL	conditioning regimens	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For all patients but 1 , conditioning regimens were based on fludarabine ( Flu ) , which was combined with other chemotherapy drugs in 50 cases ( 74 % ) and with total body irradiation ( TBI ) in 17 ( 25 % ) .
	manualset3
238045	4	427881	16	NULL	NULL	0	NULL	fludarabine ( Flu )	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	For all patients but 1 , conditioning regimens were based on fludarabine ( Flu ) , which was combined with other chemotherapy drugs in 50 cases ( 74 % ) and with total body irradiation ( TBI ) in 17 ( 25 % ) .
	manualset3
238048	5	427881	16	NULL	NULL	0	NULL	chemotherapy drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	For all patients but 1 , conditioning regimens were based on fludarabine ( Flu ) , which was combined with other chemotherapy drugs in 50 cases ( 74 % ) and with total body irradiation ( TBI ) in 17 ( 25 % ) .
	manualset3
238051	6	427881	16	NULL	NULL	0	NULL	50 cases ( 74 % )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For all patients but 1 , conditioning regimens were based on fludarabine ( Flu ) , which was combined with other chemotherapy drugs in 50 cases ( 74 % ) and with total body irradiation ( TBI ) in 17 ( 25 % ) .
	manualset3
238055	7	427881	16	NULL	NULL	0	NULL	total body irradiation ( TBI )	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For all patients but 1 , conditioning regimens were based on fludarabine ( Flu ) , which was combined with other chemotherapy drugs in 50 cases ( 74 % ) and with total body irradiation ( TBI ) in 17 ( 25 % ) .
	manualset3
238058	8	427881	16	NULL	NULL	0	NULL	17 ( 25 % )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For all patients but 1 , conditioning regimens were based on fludarabine ( Flu ) , which was combined with other chemotherapy drugs in 50 cases ( 74 % ) and with total body irradiation ( TBI ) in 17 ( 25 % ) .
	manualset3
238067	1	427882	16	NULL	NULL	0	NULL	ammonium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For ammonium , the reaction forms a blue dye ( indophenol ) with a maximum absorption at 630-650 nm .
	manualset3
238068	2	427882	16	NULL	NULL	0	NULL	reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For ammonium , the reaction forms a blue dye ( indophenol ) with a maximum absorption at 630-650 nm .
	manualset3
238069	3	427882	16	NULL	NULL	0	NULL	blue dye ( indophenol )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For ammonium , the reaction forms a blue dye ( indophenol ) with a maximum absorption at 630-650 nm .
	manualset3
238070	4	427882	16	NULL	NULL	0	NULL	absorption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For ammonium , the reaction forms a blue dye ( indophenol ) with a maximum absorption at 630-650 nm .
	manualset3
238071	5	427882	16	NULL	NULL	0	NULL	630-650 nm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For ammonium , the reaction forms a blue dye ( indophenol ) with a maximum absorption at 630-650 nm .
	manualset3
238080	1	427883	16	NULL	NULL	0	NULL	CD8 + cytotoxic T cell response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For an effective CD8 + cytotoxic T cell response to occur during infection , MHC class I molecules must be loaded with antigenic peptides in the endoplasmic reticulum .
	manualset3
238084	2	427883	16	NULL	NULL	0	NULL	infection	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For an effective CD8 + cytotoxic T cell response to occur during infection , MHC class I molecules must be loaded with antigenic peptides in the endoplasmic reticulum .
	manualset3
238088	3	427883	16	NULL	NULL	0	NULL	MHC class I molecules	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	For an effective CD8 + cytotoxic T cell response to occur during infection , MHC class I molecules must be loaded with antigenic peptides in the endoplasmic reticulum .
	manualset3
238099	4	427883	16	NULL	NULL	0	NULL	antigenic peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	For an effective CD8 + cytotoxic T cell response to occur during infection , MHC class I molecules must be loaded with antigenic peptides in the endoplasmic reticulum .
	manualset3
238102	5	427883	16	NULL	NULL	0	NULL	endoplasmic reticulum	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	For an effective CD8 + cytotoxic T cell response to occur during infection , MHC class I molecules must be loaded with antigenic peptides in the endoplasmic reticulum .
	manualset3
238131	1	427884	16	NULL	NULL	0	NULL	ASR model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	For an idealized ASR model where RLMT is active , our simulations show a discrete range of diffusive length scales over which the viability of ASR schemes in brackish aquifers would be hindered .
	manualset3
238143	2	427884	16	NULL	NULL	0	NULL	RLMT	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For an idealized ASR model where RLMT is active , our simulations show a discrete range of diffusive length scales over which the viability of ASR schemes in brackish aquifers would be hindered .
	manualset3
238146	3	427884	16	NULL	NULL	0	NULL	simulations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For an idealized ASR model where RLMT is active , our simulations show a discrete range of diffusive length scales over which the viability of ASR schemes in brackish aquifers would be hindered .
	manualset3
238149	4	427884	16	NULL	NULL	0	NULL	diffusive length scales	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For an idealized ASR model where RLMT is active , our simulations show a discrete range of diffusive length scales over which the viability of ASR schemes in brackish aquifers would be hindered .
	manualset3
238152	5	427884	16	NULL	NULL	0	NULL	viability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For an idealized ASR model where RLMT is active , our simulations show a discrete range of diffusive length scales over which the viability of ASR schemes in brackish aquifers would be hindered .
	manualset3
238153	6	427884	16	NULL	NULL	NULL	NULL	ASR schemes	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For an idealized ASR model where RLMT is active , our simulations show a discrete range of diffusive length scales over which the viability of ASR schemes in brackish aquifers would be hindered .
	manualset3
238161	7	427884	16	NULL	NULL	0	NULL	brackish aquifers	GeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	For an idealized ASR model where RLMT is active , our simulations show a discrete range of diffusive length scales over which the viability of ASR schemes in brackish aquifers would be hindered .
	manualset3
239603	8	427884	16	NULL	NULL	0	NULL	discrete range	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For an idealized ASR model where RLMT is active , our simulations show a discrete range of diffusive length scales over which the viability of ASR schemes in brackish aquifers would be hindered .
	manualset3
238164	1	427885	16	NULL	NULL	0	NULL	antibody binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For antibody binding , the full covalent structure of IFN 151-166 was required .
	manualset3
238177	2	427885	16	NULL	NULL	0	NULL	covalent structure	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For antibody binding , the full covalent structure of IFN 151-166 was required .
	manualset3
238180	3	427885	16	NULL	NULL	0	NULL	IFN 151-166	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	For antibody binding , the full covalent structure of IFN 151-166 was required .
	manualset3
238778	1	427886	16	NULL	NULL	NULL	NULL	Regulation	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Regulation of insulin secretion ) .
	manualset3
239604	2	427886	16	NULL	NULL	0	NULL	insulin secretion	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Regulation of insulin secretion ) .
	manualset3
238779	1	427887	16	NULL	NULL	0	NULL	applications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For applications in embryology , numerical estimates suggest that convection can be ignored in reaction-diffusion mechanisms for pattern formation , and this conclusion is supported by a dimensional analysis .
	manualset3
238780	2	427887	16	NULL	NULL	0	NULL	embryology	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For applications in embryology , numerical estimates suggest that convection can be ignored in reaction-diffusion mechanisms for pattern formation , and this conclusion is supported by a dimensional analysis .
	manualset3
238781	3	427887	16	NULL	NULL	0	NULL	numerical estimates	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For applications in embryology , numerical estimates suggest that convection can be ignored in reaction-diffusion mechanisms for pattern formation , and this conclusion is supported by a dimensional analysis .
	manualset3
238782	4	427887	16	NULL	NULL	0	NULL	convection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For applications in embryology , numerical estimates suggest that convection can be ignored in reaction-diffusion mechanisms for pattern formation , and this conclusion is supported by a dimensional analysis .
	manualset3
238783	5	427887	16	NULL	NULL	0	NULL	reaction-diffusion mechanisms	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For applications in embryology , numerical estimates suggest that convection can be ignored in reaction-diffusion mechanisms for pattern formation , and this conclusion is supported by a dimensional analysis .
	manualset3
238784	6	427887	16	NULL	NULL	0	NULL	pattern formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For applications in embryology , numerical estimates suggest that convection can be ignored in reaction-diffusion mechanisms for pattern formation , and this conclusion is supported by a dimensional analysis .
	manualset3
238785	7	427887	16	NULL	NULL	NULL	NULL	conclusion	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For applications in embryology , numerical estimates suggest that convection can be ignored in reaction-diffusion mechanisms for pattern formation , and this conclusion is supported by a dimensional analysis .
	manualset3
238786	8	427887	16	NULL	NULL	0	NULL	dimensional analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For applications in embryology , numerical estimates suggest that convection can be ignored in reaction-diffusion mechanisms for pattern formation , and this conclusion is supported by a dimensional analysis .
	manualset3
238787	1	427888	16	NULL	NULL	NULL	NULL	assessment	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For assessment of stenosis severity , measurement of transvalvular pressure gradient is an appropriate measure and MR may not confer benefits over echocardiography , provided the ultrasound window is adequate ( and stroke volume is in the normal range ) .
	manualset3
238788	2	427888	16	NULL	NULL	0	NULL	stenosis severity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For assessment of stenosis severity , measurement of transvalvular pressure gradient is an appropriate measure and MR may not confer benefits over echocardiography , provided the ultrasound window is adequate ( and stroke volume is in the normal range ) .
	manualset3
238789	3	427888	16	NULL	NULL	NULL	NULL	measurement	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For assessment of stenosis severity , measurement of transvalvular pressure gradient is an appropriate measure and MR may not confer benefits over echocardiography , provided the ultrasound window is adequate ( and stroke volume is in the normal range ) .
	manualset3
238790	4	427888	16	NULL	NULL	0	NULL	transvalvular pressure gradient	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For assessment of stenosis severity , measurement of transvalvular pressure gradient is an appropriate measure and MR may not confer benefits over echocardiography , provided the ultrasound window is adequate ( and stroke volume is in the normal range ) .
	manualset3
238801	5	427888	16	NULL	NULL	0	NULL	appropriate measure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For assessment of stenosis severity , measurement of transvalvular pressure gradient is an appropriate measure and MR may not confer benefits over echocardiography , provided the ultrasound window is adequate ( and stroke volume is in the normal range ) .
	manualset3
238804	6	427888	16	NULL	NULL	0	NULL	MR	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For assessment of stenosis severity , measurement of transvalvular pressure gradient is an appropriate measure and MR may not confer benefits over echocardiography , provided the ultrasound window is adequate ( and stroke volume is in the normal range ) .
	manualset3
238811	7	427888	16	NULL	NULL	0	NULL	benefits	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For assessment of stenosis severity , measurement of transvalvular pressure gradient is an appropriate measure and MR may not confer benefits over echocardiography , provided the ultrasound window is adequate ( and stroke volume is in the normal range ) .
	manualset3
238812	8	427888	16	NULL	NULL	0	NULL	echocardiography	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For assessment of stenosis severity , measurement of transvalvular pressure gradient is an appropriate measure and MR may not confer benefits over echocardiography , provided the ultrasound window is adequate ( and stroke volume is in the normal range ) .
	manualset3
238821	9	427888	16	NULL	NULL	0	NULL	ultrasound window	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For assessment of stenosis severity , measurement of transvalvular pressure gradient is an appropriate measure and MR may not confer benefits over echocardiography , provided the ultrasound window is adequate ( and stroke volume is in the normal range ) .
	manualset3
238824	10	427888	16	NULL	NULL	NULL	NULL	stroke volume	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For assessment of stenosis severity , measurement of transvalvular pressure gradient is an appropriate measure and MR may not confer benefits over echocardiography , provided the ultrasound window is adequate ( and stroke volume is in the normal range ) .
	manualset3
238826	11	427888	16	NULL	NULL	0	NULL	range	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For assessment of stenosis severity , measurement of transvalvular pressure gradient is an appropriate measure and MR may not confer benefits over echocardiography , provided the ultrasound window is adequate ( and stroke volume is in the normal range ) .
	manualset3
238835	1	427889	16	NULL	NULL	0	NULL	benzoic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For benzoic , p-chlorobenzoic and picric acids , phenylphenol and barbital , excellent recoveries were obtained from well-defined conductance vs. volume plots .
	manualset3
238836	2	427889	16	NULL	NULL	0	NULL	p-chlorobenzoic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For benzoic , p-chlorobenzoic and picric acids , phenylphenol and barbital , excellent recoveries were obtained from well-defined conductance vs. volume plots .
	manualset3
238838	3	427889	16	NULL	NULL	0	NULL	picric acids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For benzoic , p-chlorobenzoic and picric acids , phenylphenol and barbital , excellent recoveries were obtained from well-defined conductance vs. volume plots .
	manualset3
238839	4	427889	16	NULL	NULL	0	NULL	phenylphenol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For benzoic , p-chlorobenzoic and picric acids , phenylphenol and barbital , excellent recoveries were obtained from well-defined conductance vs. volume plots .
	manualset3
238840	5	427889	16	NULL	NULL	0	NULL	barbital	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For benzoic , p-chlorobenzoic and picric acids , phenylphenol and barbital , excellent recoveries were obtained from well-defined conductance vs. volume plots .
	manualset3
238946	6	427889	16	NULL	NULL	NULL	NULL	conductance vs. volume plots	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For benzoic , p-chlorobenzoic and picric acids , phenylphenol and barbital , excellent recoveries were obtained from well-defined conductance vs. volume plots .
	manualset3
239605	7	427889	16	NULL	NULL	0	NULL	recoveries	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For benzoic , p-chlorobenzoic and picric acids , phenylphenol and barbital , excellent recoveries were obtained from well-defined conductance vs. volume plots .
	manualset3
238947	1	427890	16	NULL	NULL	0	NULL	types	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For both types of leukocyte suspension labeled with In-111 oxine , the average recovery of cell-bound activity in the circulating blood at 4 hr was 32 % of the administered activity , inferior to that of DFP-32 .
	manualset3
238948	2	427890	16	NULL	NULL	0	NULL	leukocyte suspension	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	For both types of leukocyte suspension labeled with In-111 oxine , the average recovery of cell-bound activity in the circulating blood at 4 hr was 32 % of the administered activity , inferior to that of DFP-32 .
	manualset3
238950	3	427890	16	NULL	NULL	0	NULL	In-111 oxine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For both types of leukocyte suspension labeled with In-111 oxine , the average recovery of cell-bound activity in the circulating blood at 4 hr was 32 % of the administered activity , inferior to that of DFP-32 .
	manualset3
238952	4	427890	16	NULL	NULL	0	NULL	average	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For both types of leukocyte suspension labeled with In-111 oxine , the average recovery of cell-bound activity in the circulating blood at 4 hr was 32 % of the administered activity , inferior to that of DFP-32 .
	manualset3
238954	5	427890	16	NULL	NULL	0	NULL	recovery	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For both types of leukocyte suspension labeled with In-111 oxine , the average recovery of cell-bound activity in the circulating blood at 4 hr was 32 % of the administered activity , inferior to that of DFP-32 .
	manualset3
238956	6	427890	16	NULL	NULL	0	NULL	cell-bound activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For both types of leukocyte suspension labeled with In-111 oxine , the average recovery of cell-bound activity in the circulating blood at 4 hr was 32 % of the administered activity , inferior to that of DFP-32 .
	manualset3
238966	7	427890	16	NULL	NULL	NULL	NULL	circulating blood	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For both types of leukocyte suspension labeled with In-111 oxine , the average recovery of cell-bound activity in the circulating blood at 4 hr was 32 % of the administered activity , inferior to that of DFP-32 .
	manualset3
238967	8	427890	16	NULL	NULL	0	NULL	32 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For both types of leukocyte suspension labeled with In-111 oxine , the average recovery of cell-bound activity in the circulating blood at 4 hr was 32 % of the administered activity , inferior to that of DFP-32 .
	manualset3
238968	9	427890	16	NULL	NULL	NULL	NULL	administered activity	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For both types of leukocyte suspension labeled with In-111 oxine , the average recovery of cell-bound activity in the circulating blood at 4 hr was 32 % of the administered activity , inferior to that of DFP-32 .
	manualset3
238969	10	427890	16	NULL	NULL	0	NULL	inferior	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	For both types of leukocyte suspension labeled with In-111 oxine , the average recovery of cell-bound activity in the circulating blood at 4 hr was 32 % of the administered activity , inferior to that of DFP-32 .
	manualset3
238978	11	427890	16	NULL	NULL	0	NULL	DFP-32	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For both types of leukocyte suspension labeled with In-111 oxine , the average recovery of cell-bound activity in the circulating blood at 4 hr was 32 % of the administered activity , inferior to that of DFP-32 .
	manualset3
239606	12	427890	16	NULL	NULL	NULL	NULL	4 hr	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For both types of leukocyte suspension labeled with In-111 oxine , the average recovery of cell-bound activity in the circulating blood at 4 hr was 32 % of the administered activity , inferior to that of DFP-32 .
	manualset3
239014	1	427891	16	NULL	NULL	NULL	NULL	breast cancer incidence	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For breast cancer incidence , the age-period model adequately represented the data , and demonstrated that the risk of developing breast cancer has been increasing in recent time periods .
	manualset3
239017	2	427891	16	NULL	NULL	NULL	NULL	age-period model	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For breast cancer incidence , the age-period model adequately represented the data , and demonstrated that the risk of developing breast cancer has been increasing in recent time periods .
	manualset3
239018	3	427891	16	NULL	NULL	0	NULL	data	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	For breast cancer incidence , the age-period model adequately represented the data , and demonstrated that the risk of developing breast cancer has been increasing in recent time periods .
	manualset3
239019	4	427891	16	NULL	NULL	0	NULL	risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For breast cancer incidence , the age-period model adequately represented the data , and demonstrated that the risk of developing breast cancer has been increasing in recent time periods .
	manualset3
239020	5	427891	16	NULL	NULL	0	NULL	breast cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	For breast cancer incidence , the age-period model adequately represented the data , and demonstrated that the risk of developing breast cancer has been increasing in recent time periods .
	manualset3
239021	6	427891	16	NULL	NULL	0	NULL	time periods	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	For breast cancer incidence , the age-period model adequately represented the data , and demonstrated that the risk of developing breast cancer has been increasing in recent time periods .
	manualset3
239023	2	427892	16	NULL	NULL	NULL	NULL	clinical reasons	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For clinical and epidemiological reasons it is important to try to identify the culprit drug following an approach based on previous experience with the drug , timing of events , patient reaction to dechallenge , patient reaction to rechallenge ( if feasible ) , alternative aetiological candidates , and drug concentration or evidence of overdose .
	manualset3
239024	3	427892	16	NULL	NULL	NULL	NULL	epidemiological reasons	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For clinical and epidemiological reasons it is important to try to identify the culprit drug following an approach based on previous experience with the drug , timing of events , patient reaction to dechallenge , patient reaction to rechallenge ( if feasible ) , alternative aetiological candidates , and drug concentration or evidence of overdose .
	manualset3
239025	4	427892	16	NULL	NULL	0	NULL	approach	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For clinical and epidemiological reasons it is important to try to identify the culprit drug following an approach based on previous experience with the drug , timing of events , patient reaction to dechallenge , patient reaction to rechallenge ( if feasible ) , alternative aetiological candidates , and drug concentration or evidence of overdose .
	manualset3
240865	5	427892	16	NULL	NULL	0	NULL	culprit drug	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For clinical and epidemiological reasons it is important to try to identify the culprit drug following an approach based on previous experience with the drug , timing of events , patient reaction to dechallenge , patient reaction to rechallenge ( if feasible ) , alternative aetiological candidates , and drug concentration or evidence of overdose .
	manualset3
240867	6	427892	16	NULL	NULL	0	NULL	approach	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For clinical and epidemiological reasons it is important to try to identify the culprit drug following an approach based on previous experience with the drug , timing of events , patient reaction to dechallenge , patient reaction to rechallenge ( if feasible ) , alternative aetiological candidates , and drug concentration or evidence of overdose .
	manualset3
240886	7	427892	16	NULL	NULL	0	NULL	previous experience	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For clinical and epidemiological reasons it is important to try to identify the culprit drug following an approach based on previous experience with the drug , timing of events , patient reaction to dechallenge , patient reaction to rechallenge ( if feasible ) , alternative aetiological candidates , and drug concentration or evidence of overdose .
	manualset3
240890	8	427892	16	NULL	NULL	0	NULL	drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	For clinical and epidemiological reasons it is important to try to identify the culprit drug following an approach based on previous experience with the drug , timing of events , patient reaction to dechallenge , patient reaction to rechallenge ( if feasible ) , alternative aetiological candidates , and drug concentration or evidence of overdose .
	manualset3
240914	9	427892	16	NULL	NULL	0	NULL	timing of events	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	For clinical and epidemiological reasons it is important to try to identify the culprit drug following an approach based on previous experience with the drug , timing of events , patient reaction to dechallenge , patient reaction to rechallenge ( if feasible ) , alternative aetiological candidates , and drug concentration or evidence of overdose .
	manualset3
240921	10	427892	16	NULL	NULL	0	NULL	patient reaction to dechallenge	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For clinical and epidemiological reasons it is important to try to identify the culprit drug following an approach based on previous experience with the drug , timing of events , patient reaction to dechallenge , patient reaction to rechallenge ( if feasible ) , alternative aetiological candidates , and drug concentration or evidence of overdose .
	manualset3
240924	11	427892	16	NULL	NULL	0	NULL	patient reaction to rechallenge	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For clinical and epidemiological reasons it is important to try to identify the culprit drug following an approach based on previous experience with the drug , timing of events , patient reaction to dechallenge , patient reaction to rechallenge ( if feasible ) , alternative aetiological candidates , and drug concentration or evidence of overdose .
	manualset3
240927	12	427892	16	NULL	NULL	0	NULL	alternative aetiological candidates	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For clinical and epidemiological reasons it is important to try to identify the culprit drug following an approach based on previous experience with the drug , timing of events , patient reaction to dechallenge , patient reaction to rechallenge ( if feasible ) , alternative aetiological candidates , and drug concentration or evidence of overdose .
	manualset3
240928	13	427892	16	NULL	NULL	0	NULL	drug concentration	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For clinical and epidemiological reasons it is important to try to identify the culprit drug following an approach based on previous experience with the drug , timing of events , patient reaction to dechallenge , patient reaction to rechallenge ( if feasible ) , alternative aetiological candidates , and drug concentration or evidence of overdose .
	manualset3
240930	14	427892	16	NULL	NULL	0	NULL	evidence of overdose	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For clinical and epidemiological reasons it is important to try to identify the culprit drug following an approach based on previous experience with the drug , timing of events , patient reaction to dechallenge , patient reaction to rechallenge ( if feasible ) , alternative aetiological candidates , and drug concentration or evidence of overdose .
	manualset3
239026	1	427893	16	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	For comparison , parallel experiments were conducted with colchicine and taxol , two drugs active on microtubules and with tau , a structural microtubule-associated protein from brain tissue .
	manualset3
239027	2	427893	16	NULL	NULL	0	NULL	experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For comparison , parallel experiments were conducted with colchicine and taxol , two drugs active on microtubules and with tau , a structural microtubule-associated protein from brain tissue .
	manualset3
239028	3	427893	16	NULL	NULL	0	NULL	colchicine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	For comparison , parallel experiments were conducted with colchicine and taxol , two drugs active on microtubules and with tau , a structural microtubule-associated protein from brain tissue .
	manualset3
239029	4	427893	16	NULL	NULL	0	NULL	taxol	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	For comparison , parallel experiments were conducted with colchicine and taxol , two drugs active on microtubules and with tau , a structural microtubule-associated protein from brain tissue .
	manualset3
239030	5	427893	16	NULL	NULL	NULL	NULL	two drugs	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For comparison , parallel experiments were conducted with colchicine and taxol , two drugs active on microtubules and with tau , a structural microtubule-associated protein from brain tissue .
	manualset3
239031	6	427893	16	NULL	NULL	0	NULL	microtubules	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	For comparison , parallel experiments were conducted with colchicine and taxol , two drugs active on microtubules and with tau , a structural microtubule-associated protein from brain tissue .
	manualset3
239032	7	427893	16	NULL	NULL	0	NULL	tau	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For comparison , parallel experiments were conducted with colchicine and taxol , two drugs active on microtubules and with tau , a structural microtubule-associated protein from brain tissue .
	manualset3
239033	8	427893	16	NULL	NULL	0	NULL	structural microtubule-associated protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For comparison , parallel experiments were conducted with colchicine and taxol , two drugs active on microtubules and with tau , a structural microtubule-associated protein from brain tissue .
	manualset3
239034	9	427893	16	NULL	NULL	0	NULL	brain tissue	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	For comparison , parallel experiments were conducted with colchicine and taxol , two drugs active on microtubules and with tau , a structural microtubule-associated protein from brain tissue .
	manualset3
239035	1	427894	16	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	For comparison other two palladium binding polysaccharides were prepared : ( a ) a second type Pd-EPS , named Bio-Pd ( B ) , was obtained by an exchange reaction with Pd acetate starting from an iron-free EPS produced by strain BAS-10 growing on Na-citrate medium ; ( b ) a third type of palladium , named Bio-Pd ( C ) , bound to a different polysaccharide , was recovered after the same exchange reaction applied on glycolipid emulsan obtained from an aerobic culture of Acinetobacter venetianus RAG 1 .
	manualset3
239152	2	427894	16	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For comparison other two palladium binding polysaccharides were prepared : ( a ) a second type Pd-EPS , named Bio-Pd ( B ) , was obtained by an exchange reaction with Pd acetate starting from an iron-free EPS produced by strain BAS-10 growing on Na-citrate medium ; ( b ) a third type of palladium , named Bio-Pd ( C ) , bound to a different polysaccharide , was recovered after the same exchange reaction applied on glycolipid emulsan obtained from an aerobic culture of Acinetobacter venetianus RAG 1 .
	manualset3
239153	3	427894	16	NULL	NULL	0	NULL	palladium binding polysaccharides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For comparison other two palladium binding polysaccharides were prepared : ( a ) a second type Pd-EPS , named Bio-Pd ( B ) , was obtained by an exchange reaction with Pd acetate starting from an iron-free EPS produced by strain BAS-10 growing on Na-citrate medium ; ( b ) a third type of palladium , named Bio-Pd ( C ) , bound to a different polysaccharide , was recovered after the same exchange reaction applied on glycolipid emulsan obtained from an aerobic culture of Acinetobacter venetianus RAG 1 .
	manualset3
239703	4	427894	16	NULL	NULL	0	NULL	second type Pd-EPS	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For comparison other two palladium binding polysaccharides were prepared : ( a ) a second type Pd-EPS , named Bio-Pd ( B ) , was obtained by an exchange reaction with Pd acetate starting from an iron-free EPS produced by strain BAS-10 growing on Na-citrate medium ; ( b ) a third type of palladium , named Bio-Pd ( C ) , bound to a different polysaccharide , was recovered after the same exchange reaction applied on glycolipid emulsan obtained from an aerobic culture of Acinetobacter venetianus RAG 1 .
	manualset3
239704	5	427894	16	NULL	NULL	0	NULL	Bio-Pd ( B )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For comparison other two palladium binding polysaccharides were prepared : ( a ) a second type Pd-EPS , named Bio-Pd ( B ) , was obtained by an exchange reaction with Pd acetate starting from an iron-free EPS produced by strain BAS-10 growing on Na-citrate medium ; ( b ) a third type of palladium , named Bio-Pd ( C ) , bound to a different polysaccharide , was recovered after the same exchange reaction applied on glycolipid emulsan obtained from an aerobic culture of Acinetobacter venetianus RAG 1 .
	manualset3
239705	6	427894	16	NULL	NULL	0	NULL	exchange reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For comparison other two palladium binding polysaccharides were prepared : ( a ) a second type Pd-EPS , named Bio-Pd ( B ) , was obtained by an exchange reaction with Pd acetate starting from an iron-free EPS produced by strain BAS-10 growing on Na-citrate medium ; ( b ) a third type of palladium , named Bio-Pd ( C ) , bound to a different polysaccharide , was recovered after the same exchange reaction applied on glycolipid emulsan obtained from an aerobic culture of Acinetobacter venetianus RAG 1 .
	manualset3
239706	7	427894	16	NULL	NULL	0	NULL	Pd acetate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For comparison other two palladium binding polysaccharides were prepared : ( a ) a second type Pd-EPS , named Bio-Pd ( B ) , was obtained by an exchange reaction with Pd acetate starting from an iron-free EPS produced by strain BAS-10 growing on Na-citrate medium ; ( b ) a third type of palladium , named Bio-Pd ( C ) , bound to a different polysaccharide , was recovered after the same exchange reaction applied on glycolipid emulsan obtained from an aerobic culture of Acinetobacter venetianus RAG 1 .
	manualset3
239707	8	427894	16	NULL	NULL	0	NULL	iron-free EPS	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For comparison other two palladium binding polysaccharides were prepared : ( a ) a second type Pd-EPS , named Bio-Pd ( B ) , was obtained by an exchange reaction with Pd acetate starting from an iron-free EPS produced by strain BAS-10 growing on Na-citrate medium ; ( b ) a third type of palladium , named Bio-Pd ( C ) , bound to a different polysaccharide , was recovered after the same exchange reaction applied on glycolipid emulsan obtained from an aerobic culture of Acinetobacter venetianus RAG 1 .
	manualset3
239708	9	427894	16	NULL	NULL	0	NULL	strain BAS-10	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For comparison other two palladium binding polysaccharides were prepared : ( a ) a second type Pd-EPS , named Bio-Pd ( B ) , was obtained by an exchange reaction with Pd acetate starting from an iron-free EPS produced by strain BAS-10 growing on Na-citrate medium ; ( b ) a third type of palladium , named Bio-Pd ( C ) , bound to a different polysaccharide , was recovered after the same exchange reaction applied on glycolipid emulsan obtained from an aerobic culture of Acinetobacter venetianus RAG 1 .
	manualset3
239709	10	427894	16	NULL	NULL	0	NULL	Na-citrate medium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For comparison other two palladium binding polysaccharides were prepared : ( a ) a second type Pd-EPS , named Bio-Pd ( B ) , was obtained by an exchange reaction with Pd acetate starting from an iron-free EPS produced by strain BAS-10 growing on Na-citrate medium ; ( b ) a third type of palladium , named Bio-Pd ( C ) , bound to a different polysaccharide , was recovered after the same exchange reaction applied on glycolipid emulsan obtained from an aerobic culture of Acinetobacter venetianus RAG 1 .
	manualset3
239710	11	427894	16	NULL	NULL	0	NULL	third type	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For comparison other two palladium binding polysaccharides were prepared : ( a ) a second type Pd-EPS , named Bio-Pd ( B ) , was obtained by an exchange reaction with Pd acetate starting from an iron-free EPS produced by strain BAS-10 growing on Na-citrate medium ; ( b ) a third type of palladium , named Bio-Pd ( C ) , bound to a different polysaccharide , was recovered after the same exchange reaction applied on glycolipid emulsan obtained from an aerobic culture of Acinetobacter venetianus RAG 1 .
	manualset3
239711	12	427894	16	NULL	NULL	0	NULL	palladium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For comparison other two palladium binding polysaccharides were prepared : ( a ) a second type Pd-EPS , named Bio-Pd ( B ) , was obtained by an exchange reaction with Pd acetate starting from an iron-free EPS produced by strain BAS-10 growing on Na-citrate medium ; ( b ) a third type of palladium , named Bio-Pd ( C ) , bound to a different polysaccharide , was recovered after the same exchange reaction applied on glycolipid emulsan obtained from an aerobic culture of Acinetobacter venetianus RAG 1 .
	manualset3
239712	13	427894	16	NULL	NULL	0	NULL	Bio-Pd ( C )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For comparison other two palladium binding polysaccharides were prepared : ( a ) a second type Pd-EPS , named Bio-Pd ( B ) , was obtained by an exchange reaction with Pd acetate starting from an iron-free EPS produced by strain BAS-10 growing on Na-citrate medium ; ( b ) a third type of palladium , named Bio-Pd ( C ) , bound to a different polysaccharide , was recovered after the same exchange reaction applied on glycolipid emulsan obtained from an aerobic culture of Acinetobacter venetianus RAG 1 .
	manualset3
239713	14	427894	16	NULL	NULL	0	NULL	polysaccharide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For comparison other two palladium binding polysaccharides were prepared : ( a ) a second type Pd-EPS , named Bio-Pd ( B ) , was obtained by an exchange reaction with Pd acetate starting from an iron-free EPS produced by strain BAS-10 growing on Na-citrate medium ; ( b ) a third type of palladium , named Bio-Pd ( C ) , bound to a different polysaccharide , was recovered after the same exchange reaction applied on glycolipid emulsan obtained from an aerobic culture of Acinetobacter venetianus RAG 1 .
	manualset3
239714	15	427894	16	NULL	NULL	0	NULL	exchange reaction	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For comparison other two palladium binding polysaccharides were prepared : ( a ) a second type Pd-EPS , named Bio-Pd ( B ) , was obtained by an exchange reaction with Pd acetate starting from an iron-free EPS produced by strain BAS-10 growing on Na-citrate medium ; ( b ) a third type of palladium , named Bio-Pd ( C ) , bound to a different polysaccharide , was recovered after the same exchange reaction applied on glycolipid emulsan obtained from an aerobic culture of Acinetobacter venetianus RAG 1 .
	manualset3
239715	16	427894	16	NULL	NULL	0	NULL	glycolipid emulsan	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For comparison other two palladium binding polysaccharides were prepared : ( a ) a second type Pd-EPS , named Bio-Pd ( B ) , was obtained by an exchange reaction with Pd acetate starting from an iron-free EPS produced by strain BAS-10 growing on Na-citrate medium ; ( b ) a third type of palladium , named Bio-Pd ( C ) , bound to a different polysaccharide , was recovered after the same exchange reaction applied on glycolipid emulsan obtained from an aerobic culture of Acinetobacter venetianus RAG 1 .
	manualset3
239716	17	427894	16	NULL	NULL	0	NULL	aerobic culture	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For comparison other two palladium binding polysaccharides were prepared : ( a ) a second type Pd-EPS , named Bio-Pd ( B ) , was obtained by an exchange reaction with Pd acetate starting from an iron-free EPS produced by strain BAS-10 growing on Na-citrate medium ; ( b ) a third type of palladium , named Bio-Pd ( C ) , bound to a different polysaccharide , was recovered after the same exchange reaction applied on glycolipid emulsan obtained from an aerobic culture of Acinetobacter venetianus RAG 1 .
	manualset3
239717	18	427894	16	NULL	NULL	0	NULL	Acinetobacter venetianus RAG 1	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For comparison other two palladium binding polysaccharides were prepared : ( a ) a second type Pd-EPS , named Bio-Pd ( B ) , was obtained by an exchange reaction with Pd acetate starting from an iron-free EPS produced by strain BAS-10 growing on Na-citrate medium ; ( b ) a third type of palladium , named Bio-Pd ( C ) , bound to a different polysaccharide , was recovered after the same exchange reaction applied on glycolipid emulsan obtained from an aerobic culture of Acinetobacter venetianus RAG 1 .
	manualset3
239442	1	427895	16	NULL	NULL	0	NULL	strictures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For confined strictures , especially at the site of the ureteroneocystostomy , endoscopic dilation may be a good alternative .
	manualset3
239443	2	427895	16	NULL	NULL	NULL	NULL	site	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For confined strictures , especially at the site of the ureteroneocystostomy , endoscopic dilation may be a good alternative .
	manualset3
239444	3	427895	16	NULL	NULL	0	NULL	ureteroneocystostomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For confined strictures , especially at the site of the ureteroneocystostomy , endoscopic dilation may be a good alternative .
	manualset3
239445	4	427895	16	NULL	NULL	0	NULL	endoscopic dilation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For confined strictures , especially at the site of the ureteroneocystostomy , endoscopic dilation may be a good alternative .
	manualset3
239446	5	427895	16	NULL	NULL	NULL	NULL	alternative	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For confined strictures , especially at the site of the ureteroneocystostomy , endoscopic dilation may be a good alternative .
	manualset3
239447	1	427896	16	NULL	NULL	NULL	NULL	controls	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For controls , we used rats sensitized with CFA only ( Group CFA ) and untreated rats ( normal controls ) .
	manualset3
239448	2	427896	16	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For controls , we used rats sensitized with CFA only ( Group CFA ) and untreated rats ( normal controls ) .
	manualset3
239449	3	427896	16	NULL	NULL	0	NULL	CFA	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	For controls , we used rats sensitized with CFA only ( Group CFA ) and untreated rats ( normal controls ) .
	manualset3
239450	4	427896	16	NULL	NULL	0	NULL	Group CFA	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For controls , we used rats sensitized with CFA only ( Group CFA ) and untreated rats ( normal controls ) .
	manualset3
239451	5	427896	16	NULL	NULL	NULL	NULL	rats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For controls , we used rats sensitized with CFA only ( Group CFA ) and untreated rats ( normal controls ) .
	manualset3
239452	6	427896	16	NULL	NULL	NULL	NULL	normal controls	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For controls , we used rats sensitized with CFA only ( Group CFA ) and untreated rats ( normal controls ) .
	manualset3
239453	1	427897	16	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For detailed analysis , the hemagglutinin ( HA ) and neuraminidase ( NA ) genes of 27 selected Austrian H5N1 viruses originating from different regions and wild bird species were analyzed phylogenetically , which revealed two clearly separated Austrian subclusters , both belonging to European cluster EMA-1 .
	manualset3
239454	2	427897	16	NULL	NULL	0	NULL	hemagglutinin ( HA ) genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	For detailed analysis , the hemagglutinin ( HA ) and neuraminidase ( NA ) genes of 27 selected Austrian H5N1 viruses originating from different regions and wild bird species were analyzed phylogenetically , which revealed two clearly separated Austrian subclusters , both belonging to European cluster EMA-1 .
	manualset3
239455	3	427897	16	NULL	NULL	0	NULL	neuraminidase ( NA ) genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	For detailed analysis , the hemagglutinin ( HA ) and neuraminidase ( NA ) genes of 27 selected Austrian H5N1 viruses originating from different regions and wild bird species were analyzed phylogenetically , which revealed two clearly separated Austrian subclusters , both belonging to European cluster EMA-1 .
	manualset3
239456	4	427897	16	NULL	NULL	0	NULL	27	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For detailed analysis , the hemagglutinin ( HA ) and neuraminidase ( NA ) genes of 27 selected Austrian H5N1 viruses originating from different regions and wild bird species were analyzed phylogenetically , which revealed two clearly separated Austrian subclusters , both belonging to European cluster EMA-1 .
	manualset3
239457	5	427897	16	NULL	NULL	0	NULL	Austrian H5N1 viruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For detailed analysis , the hemagglutinin ( HA ) and neuraminidase ( NA ) genes of 27 selected Austrian H5N1 viruses originating from different regions and wild bird species were analyzed phylogenetically , which revealed two clearly separated Austrian subclusters , both belonging to European cluster EMA-1 .
	manualset3
239458	6	427897	16	NULL	NULL	0	NULL	regions	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	For detailed analysis , the hemagglutinin ( HA ) and neuraminidase ( NA ) genes of 27 selected Austrian H5N1 viruses originating from different regions and wild bird species were analyzed phylogenetically , which revealed two clearly separated Austrian subclusters , both belonging to European cluster EMA-1 .
	manualset3
239459	7	427897	16	NULL	NULL	0	NULL	wild bird species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For detailed analysis , the hemagglutinin ( HA ) and neuraminidase ( NA ) genes of 27 selected Austrian H5N1 viruses originating from different regions and wild bird species were analyzed phylogenetically , which revealed two clearly separated Austrian subclusters , both belonging to European cluster EMA-1 .
	manualset3
239460	8	427897	16	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For detailed analysis , the hemagglutinin ( HA ) and neuraminidase ( NA ) genes of 27 selected Austrian H5N1 viruses originating from different regions and wild bird species were analyzed phylogenetically , which revealed two clearly separated Austrian subclusters , both belonging to European cluster EMA-1 .
	manualset3
239461	9	427897	16	NULL	NULL	0	NULL	Austrian subclusters	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	For detailed analysis , the hemagglutinin ( HA ) and neuraminidase ( NA ) genes of 27 selected Austrian H5N1 viruses originating from different regions and wild bird species were analyzed phylogenetically , which revealed two clearly separated Austrian subclusters , both belonging to European cluster EMA-1 .
	manualset3
239462	10	427897	16	NULL	NULL	0	NULL	European cluster EMA-1	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	For detailed analysis , the hemagglutinin ( HA ) and neuraminidase ( NA ) genes of 27 selected Austrian H5N1 viruses originating from different regions and wild bird species were analyzed phylogenetically , which revealed two clearly separated Austrian subclusters , both belonging to European cluster EMA-1 .
	manualset3
239719	2	427898	16	NULL	NULL	0	NULL	wrist bone	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	For each individual wrist bone we recorded the incidence of fractures , clinical treatment and diagnoses , including any special x-ray takes that would be necessary for the detection of a particular fracture .
	manualset3
239720	3	427898	16	NULL	NULL	0	NULL	incidence	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For each individual wrist bone we recorded the incidence of fractures , clinical treatment and diagnoses , including any special x-ray takes that would be necessary for the detection of a particular fracture .
	manualset3
239721	4	427898	16	NULL	NULL	0	NULL	fractures	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For each individual wrist bone we recorded the incidence of fractures , clinical treatment and diagnoses , including any special x-ray takes that would be necessary for the detection of a particular fracture .
	manualset3
239722	5	427898	16	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For each individual wrist bone we recorded the incidence of fractures , clinical treatment and diagnoses , including any special x-ray takes that would be necessary for the detection of a particular fracture .
	manualset3
239723	6	427898	16	NULL	NULL	0	NULL	diagnoses	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For each individual wrist bone we recorded the incidence of fractures , clinical treatment and diagnoses , including any special x-ray takes that would be necessary for the detection of a particular fracture .
	manualset3
239724	7	427898	16	NULL	NULL	NULL	NULL	x-ray takes	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For each individual wrist bone we recorded the incidence of fractures , clinical treatment and diagnoses , including any special x-ray takes that would be necessary for the detection of a particular fracture .
	manualset3
239725	8	427898	16	NULL	NULL	0	NULL	detection	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For each individual wrist bone we recorded the incidence of fractures , clinical treatment and diagnoses , including any special x-ray takes that would be necessary for the detection of a particular fracture .
	manualset3
239726	9	427898	16	NULL	NULL	0	NULL	fracture	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For each individual wrist bone we recorded the incidence of fractures , clinical treatment and diagnoses , including any special x-ray takes that would be necessary for the detection of a particular fracture .
	manualset3
239727	1	427899	16	NULL	NULL	NULL	NULL	intervention	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For each intervention , the costs and clinical outcomes associated with that strategy must be compared with an alternate strategy for treating the same patients .
	manualset3
239728	2	427899	16	NULL	NULL	0	NULL	costs	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For each intervention , the costs and clinical outcomes associated with that strategy must be compared with an alternate strategy for treating the same patients .
	manualset3
239729	3	427899	16	NULL	NULL	0	NULL	clinical outcomes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For each intervention , the costs and clinical outcomes associated with that strategy must be compared with an alternate strategy for treating the same patients .
	manualset3
239730	4	427899	16	NULL	NULL	0	NULL	strategy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For each intervention , the costs and clinical outcomes associated with that strategy must be compared with an alternate strategy for treating the same patients .
	manualset3
239731	5	427899	16	NULL	NULL	0	NULL	strategy	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For each intervention , the costs and clinical outcomes associated with that strategy must be compared with an alternate strategy for treating the same patients .
	manualset3
239732	6	427899	16	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	For each intervention , the costs and clinical outcomes associated with that strategy must be compared with an alternate strategy for treating the same patients .
	manualset3
243021	7	427899	16	NULL	NULL	0	NULL	treating	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For each intervention , the costs and clinical outcomes associated with that strategy must be compared with an alternate strategy for treating the same patients .
	manualset3
239733	1	427900	16	NULL	NULL	0	NULL	measurement	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For each measurement , the variability and standard errors at each site appear greater for CF and FP ( 24 % ) , than for SCR ( 14 % ) .
	manualset3
239734	2	427900	16	NULL	NULL	0	NULL	variability	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For each measurement , the variability and standard errors at each site appear greater for CF and FP ( 24 % ) , than for SCR ( 14 % ) .
	manualset3
239735	3	427900	16	NULL	NULL	0	NULL	standard errors	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For each measurement , the variability and standard errors at each site appear greater for CF and FP ( 24 % ) , than for SCR ( 14 % ) .
	manualset3
239736	4	427900	16	NULL	NULL	0	NULL	site	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For each measurement , the variability and standard errors at each site appear greater for CF and FP ( 24 % ) , than for SCR ( 14 % ) .
	manualset3
239737	5	427900	16	NULL	NULL	0	NULL	CF	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For each measurement , the variability and standard errors at each site appear greater for CF and FP ( 24 % ) , than for SCR ( 14 % ) .
	manualset3
239738	6	427900	16	NULL	NULL	0	NULL	FP	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For each measurement , the variability and standard errors at each site appear greater for CF and FP ( 24 % ) , than for SCR ( 14 % ) .
	manualset3
239739	7	427900	16	NULL	NULL	0	NULL	24 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For each measurement , the variability and standard errors at each site appear greater for CF and FP ( 24 % ) , than for SCR ( 14 % ) .
	manualset3
239740	8	427900	16	NULL	NULL	0	NULL	SCR	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For each measurement , the variability and standard errors at each site appear greater for CF and FP ( 24 % ) , than for SCR ( 14 % ) .
	manualset3
239741	9	427900	16	NULL	NULL	0	NULL	14 %	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For each measurement , the variability and standard errors at each site appear greater for CF and FP ( 24 % ) , than for SCR ( 14 % ) .
	manualset3
239742	1	427901	16	NULL	NULL	0	NULL	Reimplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Reimplantation of the common bile duct and pancreatic duct into the duodenal stump ) .
	manualset3
239743	2	427901	16	NULL	NULL	0	NULL	common bile duct	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Reimplantation of the common bile duct and pancreatic duct into the duodenal stump ) .
	manualset3
239744	3	427901	16	NULL	NULL	NULL	NULL	pancreatic duct	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Reimplantation of the common bile duct and pancreatic duct into the duodenal stump ) .
	manualset3
239745	4	427901	16	NULL	NULL	0	NULL	duodenal stump	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Reimplantation of the common bile duct and pancreatic duct into the duodenal stump ) .
	manualset3
239784	1	427902	16	NULL	NULL	0	NULL	neuronal network	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	For each type of neuronal network , the variation properties of synaptic weights are examined first .
	manualset3
239785	2	427902	16	NULL	NULL	NULL	NULL	variation properties	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For each type of neuronal network , the variation properties of synaptic weights are examined first .
	manualset3
239794	4	427902	16	NULL	NULL	0	NULL	synaptic weights	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For each type of neuronal network , the variation properties of synaptic weights are examined first .
	manualset3
239803	1	427903	16	NULL	NULL	NULL	NULL	energy calibration purposes	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For energy and fluence calibration purposes , measurements were performed with the accelerator for metrology and neutron applications in external dosimetry ( AMANDE ) facility at the Laboratory of Neutron Metrology and Dosimetry ( Institute of Radiation Protection and Nuclear Safety , IRSN , France ) .
	manualset3
239805	2	427903	16	NULL	NULL	NULL	NULL	fluence calibration purposes	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For energy and fluence calibration purposes , measurements were performed with the accelerator for metrology and neutron applications in external dosimetry ( AMANDE ) facility at the Laboratory of Neutron Metrology and Dosimetry ( Institute of Radiation Protection and Nuclear Safety , IRSN , France ) .
	manualset3
239812	4	427903	16	NULL	NULL	0	NULL	measurements	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For energy and fluence calibration purposes , measurements were performed with the accelerator for metrology and neutron applications in external dosimetry ( AMANDE ) facility at the Laboratory of Neutron Metrology and Dosimetry ( Institute of Radiation Protection and Nuclear Safety , IRSN , France ) .
	manualset3
239816	5	427903	16	NULL	NULL	0	NULL	accelerator for metrology and neutron applications in external dosimetry ( AMANDE ) facility	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	For energy and fluence calibration purposes , measurements were performed with the accelerator for metrology and neutron applications in external dosimetry ( AMANDE ) facility at the Laboratory of Neutron Metrology and Dosimetry ( Institute of Radiation Protection and Nuclear Safety , IRSN , France ) .
	manualset3
239818	6	427903	16	NULL	NULL	0	NULL	Laboratory of Neutron Metrology and Dosimetry	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	For energy and fluence calibration purposes , measurements were performed with the accelerator for metrology and neutron applications in external dosimetry ( AMANDE ) facility at the Laboratory of Neutron Metrology and Dosimetry ( Institute of Radiation Protection and Nuclear Safety , IRSN , France ) .
	manualset3
239820	7	427903	16	NULL	NULL	NULL	NULL	Institute of Radiation Protection and Nuclear Safety , IRSN	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For energy and fluence calibration purposes , measurements were performed with the accelerator for metrology and neutron applications in external dosimetry ( AMANDE ) facility at the Laboratory of Neutron Metrology and Dosimetry ( Institute of Radiation Protection and Nuclear Safety , IRSN , France ) .
	manualset3
239824	8	427903	16	NULL	NULL	0	NULL	France	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	For energy and fluence calibration purposes , measurements were performed with the accelerator for metrology and neutron applications in external dosimetry ( AMANDE ) facility at the Laboratory of Neutron Metrology and Dosimetry ( Institute of Radiation Protection and Nuclear Safety , IRSN , France ) .
	manualset3
239827	1	427904	16	NULL	NULL	NULL	NULL	evolutionists	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For evolutionists , the tree was a tool to understand the past of known ( cultured ) organisms , mapping the invention of various physiologies on the evolutionary history of microbes .
	manualset3
239864	2	427904	16	NULL	NULL	0	NULL	tree	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	For evolutionists , the tree was a tool to understand the past of known ( cultured ) organisms , mapping the invention of various physiologies on the evolutionary history of microbes .
	manualset3
239868	3	427904	16	NULL	NULL	0	NULL	tool	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For evolutionists , the tree was a tool to understand the past of known ( cultured ) organisms , mapping the invention of various physiologies on the evolutionary history of microbes .
	manualset3
239890	4	427904	16	NULL	NULL	0	NULL	past	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For evolutionists , the tree was a tool to understand the past of known ( cultured ) organisms , mapping the invention of various physiologies on the evolutionary history of microbes .
	manualset3
239892	5	427904	16	NULL	NULL	0	NULL	organisms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For evolutionists , the tree was a tool to understand the past of known ( cultured ) organisms , mapping the invention of various physiologies on the evolutionary history of microbes .
	manualset3
239905	6	427904	16	NULL	NULL	0	NULL	invention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For evolutionists , the tree was a tool to understand the past of known ( cultured ) organisms , mapping the invention of various physiologies on the evolutionary history of microbes .
	manualset3
239940	7	427904	16	NULL	NULL	0	NULL	physiologies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For evolutionists , the tree was a tool to understand the past of known ( cultured ) organisms , mapping the invention of various physiologies on the evolutionary history of microbes .
	manualset3
239941	8	427904	16	NULL	NULL	0	NULL	history	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For evolutionists , the tree was a tool to understand the past of known ( cultured ) organisms , mapping the invention of various physiologies on the evolutionary history of microbes .
	manualset3
239942	9	427904	16	NULL	NULL	0	NULL	microbes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For evolutionists , the tree was a tool to understand the past of known ( cultured ) organisms , mapping the invention of various physiologies on the evolutionary history of microbes .
	manualset3
240109	2	427905	16	NULL	NULL	0	NULL	Arabidopsis thaliana	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , Arabidopsis thaliana contains one G , one G , three G , and one RGS protein .
	manualset3
240113	3	427905	16	NULL	NULL	0	NULL	one G protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , Arabidopsis thaliana contains one G , one G , three G , and one RGS protein .
	manualset3
240115	4	427905	16	NULL	NULL	0	NULL	one G protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , Arabidopsis thaliana contains one G , one G , three G , and one RGS protein .
	manualset3
240119	5	427905	16	NULL	NULL	0	NULL	three G protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , Arabidopsis thaliana contains one G , one G , three G , and one RGS protein .
	manualset3
240122	6	427905	16	NULL	NULL	0	NULL	one RGS protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , Arabidopsis thaliana contains one G , one G , three G , and one RGS protein .
	manualset3
240126	2	427906	16	NULL	NULL	0	NULL	Burkholderia cepacia EC-K014	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , Burkholderia cepacia EC-K014 , originally isolated from the rhizoplane of a Melastoma sp. , could grow even in Mg ( 2 + ) - free Hoagland 's no. 2 medium with saccharose and glutamine ( HSG medium ) and requires a trace level of Mg ( 2 + ) for its growth .
	manualset3
240127	3	427906	16	NULL	NULL	0	NULL	rhizoplane	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , Burkholderia cepacia EC-K014 , originally isolated from the rhizoplane of a Melastoma sp. , could grow even in Mg ( 2 + ) - free Hoagland 's no. 2 medium with saccharose and glutamine ( HSG medium ) and requires a trace level of Mg ( 2 + ) for its growth .
	manualset3
240128	4	427906	16	NULL	NULL	0	NULL	Melastoma sp.	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , Burkholderia cepacia EC-K014 , originally isolated from the rhizoplane of a Melastoma sp. , could grow even in Mg ( 2 + ) - free Hoagland 's no. 2 medium with saccharose and glutamine ( HSG medium ) and requires a trace level of Mg ( 2 + ) for its growth .
	manualset3
240129	5	427906	16	NULL	NULL	0	NULL	Mg ( 2 + )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , Burkholderia cepacia EC-K014 , originally isolated from the rhizoplane of a Melastoma sp. , could grow even in Mg ( 2 + ) - free Hoagland 's no. 2 medium with saccharose and glutamine ( HSG medium ) and requires a trace level of Mg ( 2 + ) for its growth .
	manualset3
240130	6	427906	16	NULL	NULL	0	NULL	Hoagland 's no. 2 medium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , Burkholderia cepacia EC-K014 , originally isolated from the rhizoplane of a Melastoma sp. , could grow even in Mg ( 2 + ) - free Hoagland 's no. 2 medium with saccharose and glutamine ( HSG medium ) and requires a trace level of Mg ( 2 + ) for its growth .
	manualset3
240131	7	427906	16	NULL	NULL	0	NULL	saccharose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , Burkholderia cepacia EC-K014 , originally isolated from the rhizoplane of a Melastoma sp. , could grow even in Mg ( 2 + ) - free Hoagland 's no. 2 medium with saccharose and glutamine ( HSG medium ) and requires a trace level of Mg ( 2 + ) for its growth .
	manualset3
240132	8	427906	16	NULL	NULL	0	NULL	glutamine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , Burkholderia cepacia EC-K014 , originally isolated from the rhizoplane of a Melastoma sp. , could grow even in Mg ( 2 + ) - free Hoagland 's no. 2 medium with saccharose and glutamine ( HSG medium ) and requires a trace level of Mg ( 2 + ) for its growth .
	manualset3
240133	9	427906	16	NULL	NULL	0	NULL	HSG medium	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , Burkholderia cepacia EC-K014 , originally isolated from the rhizoplane of a Melastoma sp. , could grow even in Mg ( 2 + ) - free Hoagland 's no. 2 medium with saccharose and glutamine ( HSG medium ) and requires a trace level of Mg ( 2 + ) for its growth .
	manualset3
240134	10	427906	16	NULL	NULL	0	NULL	trace level	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , Burkholderia cepacia EC-K014 , originally isolated from the rhizoplane of a Melastoma sp. , could grow even in Mg ( 2 + ) - free Hoagland 's no. 2 medium with saccharose and glutamine ( HSG medium ) and requires a trace level of Mg ( 2 + ) for its growth .
	manualset3
240136	11	427906	16	NULL	NULL	0	NULL	Mg ( 2 + )	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , Burkholderia cepacia EC-K014 , originally isolated from the rhizoplane of a Melastoma sp. , could grow even in Mg ( 2 + ) - free Hoagland 's no. 2 medium with saccharose and glutamine ( HSG medium ) and requires a trace level of Mg ( 2 + ) for its growth .
	manualset3
240229	12	427906	16	NULL	NULL	0	NULL	growth	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , Burkholderia cepacia EC-K014 , originally isolated from the rhizoplane of a Melastoma sp. , could grow even in Mg ( 2 + ) - free Hoagland 's no. 2 medium with saccharose and glutamine ( HSG medium ) and requires a trace level of Mg ( 2 + ) for its growth .
	manualset3
240138	2	427907	16	NULL	NULL	0	NULL	S100A8	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , S100A8 and S100A9 ( S100A8/A9 ) have both intracellular and extracellular actions , they are abundantly expressed in inflammatory and autoimmune states , primarily by myeloid cells but also by other vascular cells , and they modulate inflammatory processes , in part through Toll-like receptor 4 and the receptor for advanced glycation end products .
	manualset3
240139	3	427907	16	NULL	NULL	0	NULL	S100A9	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , S100A8 and S100A9 ( S100A8/A9 ) have both intracellular and extracellular actions , they are abundantly expressed in inflammatory and autoimmune states , primarily by myeloid cells but also by other vascular cells , and they modulate inflammatory processes , in part through Toll-like receptor 4 and the receptor for advanced glycation end products .
	manualset3
240140	4	427907	16	NULL	NULL	0	NULL	S100A8/A9	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , S100A8 and S100A9 ( S100A8/A9 ) have both intracellular and extracellular actions , they are abundantly expressed in inflammatory and autoimmune states , primarily by myeloid cells but also by other vascular cells , and they modulate inflammatory processes , in part through Toll-like receptor 4 and the receptor for advanced glycation end products .
	manualset3
240141	5	427907	16	NULL	NULL	0	NULL	intracellular actions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , S100A8 and S100A9 ( S100A8/A9 ) have both intracellular and extracellular actions , they are abundantly expressed in inflammatory and autoimmune states , primarily by myeloid cells but also by other vascular cells , and they modulate inflammatory processes , in part through Toll-like receptor 4 and the receptor for advanced glycation end products .
	manualset3
240142	6	427907	16	NULL	NULL	0	NULL	extracellular actions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , S100A8 and S100A9 ( S100A8/A9 ) have both intracellular and extracellular actions , they are abundantly expressed in inflammatory and autoimmune states , primarily by myeloid cells but also by other vascular cells , and they modulate inflammatory processes , in part through Toll-like receptor 4 and the receptor for advanced glycation end products .
	manualset3
240143	7	427907	16	NULL	NULL	0	NULL	inflammatory states	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , S100A8 and S100A9 ( S100A8/A9 ) have both intracellular and extracellular actions , they are abundantly expressed in inflammatory and autoimmune states , primarily by myeloid cells but also by other vascular cells , and they modulate inflammatory processes , in part through Toll-like receptor 4 and the receptor for advanced glycation end products .
	manualset3
240144	8	427907	16	NULL	NULL	0	NULL	autoimmune states	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , S100A8 and S100A9 ( S100A8/A9 ) have both intracellular and extracellular actions , they are abundantly expressed in inflammatory and autoimmune states , primarily by myeloid cells but also by other vascular cells , and they modulate inflammatory processes , in part through Toll-like receptor 4 and the receptor for advanced glycation end products .
	manualset3
240145	9	427907	16	NULL	NULL	0	NULL	myeloid cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , S100A8 and S100A9 ( S100A8/A9 ) have both intracellular and extracellular actions , they are abundantly expressed in inflammatory and autoimmune states , primarily by myeloid cells but also by other vascular cells , and they modulate inflammatory processes , in part through Toll-like receptor 4 and the receptor for advanced glycation end products .
	manualset3
240146	10	427907	16	NULL	NULL	0	NULL	vascular cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , S100A8 and S100A9 ( S100A8/A9 ) have both intracellular and extracellular actions , they are abundantly expressed in inflammatory and autoimmune states , primarily by myeloid cells but also by other vascular cells , and they modulate inflammatory processes , in part through Toll-like receptor 4 and the receptor for advanced glycation end products .
	manualset3
240147	11	427907	16	NULL	NULL	0	NULL	inflammatory processes	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , S100A8 and S100A9 ( S100A8/A9 ) have both intracellular and extracellular actions , they are abundantly expressed in inflammatory and autoimmune states , primarily by myeloid cells but also by other vascular cells , and they modulate inflammatory processes , in part through Toll-like receptor 4 and the receptor for advanced glycation end products .
	manualset3
240148	12	427907	16	NULL	NULL	0	NULL	Toll-like receptor 4	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , S100A8 and S100A9 ( S100A8/A9 ) have both intracellular and extracellular actions , they are abundantly expressed in inflammatory and autoimmune states , primarily by myeloid cells but also by other vascular cells , and they modulate inflammatory processes , in part through Toll-like receptor 4 and the receptor for advanced glycation end products .
	manualset3
240149	13	427907	16	NULL	NULL	0	NULL	receptor for advanced glycation end products	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , S100A8 and S100A9 ( S100A8/A9 ) have both intracellular and extracellular actions , they are abundantly expressed in inflammatory and autoimmune states , primarily by myeloid cells but also by other vascular cells , and they modulate inflammatory processes , in part through Toll-like receptor 4 and the receptor for advanced glycation end products .
	manualset3
239022	1	427908	16	NULL	NULL	NULL	NULL	bird	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For example , a child may acquire the rule `` If it has wings , then it is a bird , '' but then must account for exceptions to this rule , such as bats .
	manualset3
240231	2	427908	16	NULL	NULL	0	NULL	child	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , a child may acquire the rule `` If it has wings , then it is a bird , '' but then must account for exceptions to this rule , such as bats .
	manualset3
240232	3	427908	16	NULL	NULL	0	NULL	rule	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , a child may acquire the rule `` If it has wings , then it is a bird , '' but then must account for exceptions to this rule , such as bats .
	manualset3
240233	4	427908	16	NULL	NULL	0	NULL	wings	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , a child may acquire the rule `` If it has wings , then it is a bird , '' but then must account for exceptions to this rule , such as bats .
	manualset3
240508	6	427908	16	NULL	NULL	NULL	NULL	exceptions	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For example , a child may acquire the rule `` If it has wings , then it is a bird , '' but then must account for exceptions to this rule , such as bats .
	manualset3
240510	7	427908	16	NULL	NULL	NULL	NULL	rule	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For example , a child may acquire the rule `` If it has wings , then it is a bird , '' but then must account for exceptions to this rule , such as bats .
	manualset3
240511	8	427908	16	NULL	NULL	0	NULL	bats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , a child may acquire the rule `` If it has wings , then it is a bird , '' but then must account for exceptions to this rule , such as bats .
	manualset3
240763	2	427909	16	NULL	NULL	0	NULL	bacterial infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , bacterial and viral infections may precipitate autoimmune disease in genetically susceptible individuals by exposing autoreactive T cells to cross-reactive peptides ( molecular mimicry ) or by enhancing lymphocyte stimulation .
	manualset3
240764	3	427909	16	NULL	NULL	0	NULL	viral infections	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , bacterial and viral infections may precipitate autoimmune disease in genetically susceptible individuals by exposing autoreactive T cells to cross-reactive peptides ( molecular mimicry ) or by enhancing lymphocyte stimulation .
	manualset3
240770	4	427909	16	NULL	NULL	0	NULL	autoimmune disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , bacterial and viral infections may precipitate autoimmune disease in genetically susceptible individuals by exposing autoreactive T cells to cross-reactive peptides ( molecular mimicry ) or by enhancing lymphocyte stimulation .
	manualset3
240771	5	427909	16	NULL	NULL	0	NULL	genetically susceptible individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , bacterial and viral infections may precipitate autoimmune disease in genetically susceptible individuals by exposing autoreactive T cells to cross-reactive peptides ( molecular mimicry ) or by enhancing lymphocyte stimulation .
	manualset3
240772	6	427909	16	NULL	NULL	0	NULL	autoreactive T cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , bacterial and viral infections may precipitate autoimmune disease in genetically susceptible individuals by exposing autoreactive T cells to cross-reactive peptides ( molecular mimicry ) or by enhancing lymphocyte stimulation .
	manualset3
240773	7	427909	16	NULL	NULL	0	NULL	cross-reactive peptides	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , bacterial and viral infections may precipitate autoimmune disease in genetically susceptible individuals by exposing autoreactive T cells to cross-reactive peptides ( molecular mimicry ) or by enhancing lymphocyte stimulation .
	manualset3
240780	8	427909	16	NULL	NULL	0	NULL	molecular mimicry	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , bacterial and viral infections may precipitate autoimmune disease in genetically susceptible individuals by exposing autoreactive T cells to cross-reactive peptides ( molecular mimicry ) or by enhancing lymphocyte stimulation .
	manualset3
240789	9	427909	16	NULL	NULL	0	NULL	lymphocyte stimulation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , bacterial and viral infections may precipitate autoimmune disease in genetically susceptible individuals by exposing autoreactive T cells to cross-reactive peptides ( molecular mimicry ) or by enhancing lymphocyte stimulation .
	manualset3
240800	2	427910	16	NULL	NULL	0	NULL	drosopterin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , drosopterin concentration correlated significantly with red chroma in the male 's dewlap center .
	manualset3
240803	3	427910	16	NULL	NULL	0	NULL	concentration	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , drosopterin concentration correlated significantly with red chroma in the male 's dewlap center .
	manualset3
240805	4	427910	16	NULL	NULL	0	NULL	red chroma	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , drosopterin concentration correlated significantly with red chroma in the male 's dewlap center .
	manualset3
240807	5	427910	16	NULL	NULL	0	NULL	male	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , drosopterin concentration correlated significantly with red chroma in the male 's dewlap center .
	manualset3
240810	6	427910	16	NULL	NULL	0	NULL	dewlap center	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , drosopterin concentration correlated significantly with red chroma in the male 's dewlap center .
	manualset3
240818	1	427911	16	NULL	NULL	0	NULL	Relation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relation between novocaine injection in cervical region and carotid sinus ; animal experimental studies ) .
	manualset3
240823	2	427911	16	NULL	NULL	0	NULL	novocaine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relation between novocaine injection in cervical region and carotid sinus ; animal experimental studies ) .
	manualset3
240827	3	427911	16	NULL	NULL	0	NULL	injection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relation between novocaine injection in cervical region and carotid sinus ; animal experimental studies ) .
	manualset3
240831	4	427911	16	NULL	NULL	0	NULL	cervical region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relation between novocaine injection in cervical region and carotid sinus ; animal experimental studies ) .
	manualset3
240833	5	427911	16	NULL	NULL	0	NULL	carotid sinus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relation between novocaine injection in cervical region and carotid sinus ; animal experimental studies ) .
	manualset3
240835	6	427911	16	NULL	NULL	0	NULL	animal experimental studies	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relation between novocaine injection in cervical region and carotid sinus ; animal experimental studies ) .
	manualset3
241212	2	427912	16	NULL	NULL	0	NULL	glutamate	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , glutamate application to motoneuronal cultures has been reported to modulate neurite formation in some studies while in others it has been reported to kill cells .
	manualset3
241213	3	427912	16	NULL	NULL	0	NULL	application	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , glutamate application to motoneuronal cultures has been reported to modulate neurite formation in some studies while in others it has been reported to kill cells .
	manualset3
241214	4	427912	16	NULL	NULL	0	NULL	motoneuronal cultures	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , glutamate application to motoneuronal cultures has been reported to modulate neurite formation in some studies while in others it has been reported to kill cells .
	manualset3
241215	5	427912	16	NULL	NULL	0	NULL	neurite formation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , glutamate application to motoneuronal cultures has been reported to modulate neurite formation in some studies while in others it has been reported to kill cells .
	manualset3
241216	6	427912	16	NULL	NULL	NULL	NULL	studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For example , glutamate application to motoneuronal cultures has been reported to modulate neurite formation in some studies while in others it has been reported to kill cells .
	manualset3
241217	7	427912	16	NULL	NULL	NULL	NULL	cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For example , glutamate application to motoneuronal cultures has been reported to modulate neurite formation in some studies while in others it has been reported to kill cells .
	manualset3
241219	2	427913	16	NULL	NULL	0	NULL	high-temperature	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , high-temperature creep-resistant ferritic steels achieve optimal creep strength ( at 923 K ) through the dispersion of yttrium oxide nanoparticles .
	manualset3
241220	3	427913	16	NULL	NULL	0	NULL	creep-resistant ferritic steels	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , high-temperature creep-resistant ferritic steels achieve optimal creep strength ( at 923 K ) through the dispersion of yttrium oxide nanoparticles .
	manualset3
241221	4	427913	16	NULL	NULL	0	NULL	creep strength	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , high-temperature creep-resistant ferritic steels achieve optimal creep strength ( at 923 K ) through the dispersion of yttrium oxide nanoparticles .
	manualset3
241222	5	427913	16	NULL	NULL	0	NULL	923 K	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , high-temperature creep-resistant ferritic steels achieve optimal creep strength ( at 923 K ) through the dispersion of yttrium oxide nanoparticles .
	manualset3
241223	6	427913	16	NULL	NULL	NULL	NULL	dispersion	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For example , high-temperature creep-resistant ferritic steels achieve optimal creep strength ( at 923 K ) through the dispersion of yttrium oxide nanoparticles .
	manualset3
241224	7	427913	16	NULL	NULL	0	NULL	yttrium oxide nanoparticles	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , high-temperature creep-resistant ferritic steels achieve optimal creep strength ( at 923 K ) through the dispersion of yttrium oxide nanoparticles .
	manualset3
241226	2	427914	16	NULL	NULL	0	NULL	1977	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , in 1977 , only 6600 men of a total of 200 , 000 under contraception have used vasectomy .
	manualset3
241228	4	427914	16	NULL	NULL	NULL	NULL	6600 men	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For example , in 1977 , only 6600 men of a total of 200 , 000 under contraception have used vasectomy .
	manualset3
241229	5	427914	16	NULL	NULL	NULL	NULL	200 , 000 men	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For example , in 1977 , only 6600 men of a total of 200 , 000 under contraception have used vasectomy .
	manualset3
241230	6	427914	16	NULL	NULL	0	NULL	contraception	MedicalProcedureOrDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , in 1977 , only 6600 men of a total of 200 , 000 under contraception have used vasectomy .
	manualset3
241231	7	427914	16	NULL	NULL	0	NULL	vasectomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , in 1977 , only 6600 men of a total of 200 , 000 under contraception have used vasectomy .
	manualset3
241234	3	427915	16	NULL	NULL	NULL	NULL	experimental finding	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For example , one can assess a recent experimental , clinical or epidemiologic finding that connects two disparate fields of inquiry -- identifying likely mechanisms to explain the finding , and choosing promising follow-up lines of investigation .
	manualset3
241235	4	427915	16	NULL	NULL	0	NULL	clinical finding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , one can assess a recent experimental , clinical or epidemiologic finding that connects two disparate fields of inquiry -- identifying likely mechanisms to explain the finding , and choosing promising follow-up lines of investigation .
	manualset3
241236	5	427915	16	NULL	NULL	0	NULL	epidemiologic finding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , one can assess a recent experimental , clinical or epidemiologic finding that connects two disparate fields of inquiry -- identifying likely mechanisms to explain the finding , and choosing promising follow-up lines of investigation .
	manualset3
241237	6	427915	16	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , one can assess a recent experimental , clinical or epidemiologic finding that connects two disparate fields of inquiry -- identifying likely mechanisms to explain the finding , and choosing promising follow-up lines of investigation .
	manualset3
241239	8	427915	16	NULL	NULL	NULL	NULL	fields of inquiry	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For example , one can assess a recent experimental , clinical or epidemiologic finding that connects two disparate fields of inquiry -- identifying likely mechanisms to explain the finding , and choosing promising follow-up lines of investigation .
	manualset3
241240	9	427915	16	NULL	NULL	0	NULL	mechanisms	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , one can assess a recent experimental , clinical or epidemiologic finding that connects two disparate fields of inquiry -- identifying likely mechanisms to explain the finding , and choosing promising follow-up lines of investigation .
	manualset3
241241	10	427915	16	NULL	NULL	0	NULL	finding	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , one can assess a recent experimental , clinical or epidemiologic finding that connects two disparate fields of inquiry -- identifying likely mechanisms to explain the finding , and choosing promising follow-up lines of investigation .
	manualset3
241242	11	427915	16	NULL	NULL	NULL	NULL	follow-up lines	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For example , one can assess a recent experimental , clinical or epidemiologic finding that connects two disparate fields of inquiry -- identifying likely mechanisms to explain the finding , and choosing promising follow-up lines of investigation .
	manualset3
241243	12	427915	16	NULL	NULL	NULL	NULL	investigation	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For example , one can assess a recent experimental , clinical or epidemiologic finding that connects two disparate fields of inquiry -- identifying likely mechanisms to explain the finding , and choosing promising follow-up lines of investigation .
	manualset3
241750	2	427916	16	NULL	NULL	0	NULL	samples	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , samples inoculated with sewage were correctly identified as containing human fecal contamination because they contained human adenovirus or human enterovirus .
	manualset3
241753	3	427916	16	NULL	NULL	0	NULL	sewage	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , samples inoculated with sewage were correctly identified as containing human fecal contamination because they contained human adenovirus or human enterovirus .
	manualset3
241754	4	427916	16	NULL	NULL	0	NULL	human fecal contamination	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , samples inoculated with sewage were correctly identified as containing human fecal contamination because they contained human adenovirus or human enterovirus .
	manualset3
241755	5	427916	16	NULL	NULL	0	NULL	human adenovirus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , samples inoculated with sewage were correctly identified as containing human fecal contamination because they contained human adenovirus or human enterovirus .
	manualset3
241756	6	427916	16	NULL	NULL	0	NULL	human enterovirus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , samples inoculated with sewage were correctly identified as containing human fecal contamination because they contained human adenovirus or human enterovirus .
	manualset3
241807	3	427917	16	NULL	NULL	0	NULL	candy	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , when instructed to click the `` candy , '' participants ' mouse-cursor trajectories curved conspicuously toward a picture of a candle before landing on the picture of the candy .
	manualset3
241808	4	427917	16	NULL	NULL	0	NULL	participants	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , when instructed to click the `` candy , '' participants ' mouse-cursor trajectories curved conspicuously toward a picture of a candle before landing on the picture of the candy .
	manualset3
241809	5	427917	16	NULL	NULL	0	NULL	mouse-cursor trajectories	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For example , when instructed to click the `` candy , '' participants ' mouse-cursor trajectories curved conspicuously toward a picture of a candle before landing on the picture of the candy .
	manualset3
241810	6	427917	16	NULL	NULL	NULL	NULL	picture of candy	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For example , when instructed to click the `` candy , '' participants ' mouse-cursor trajectories curved conspicuously toward a picture of a candle before landing on the picture of the candy .
	manualset3
241811	7	427917	16	NULL	NULL	NULL	NULL	picture of candle	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For example , when instructed to click the `` candy , '' participants ' mouse-cursor trajectories curved conspicuously toward a picture of a candle before landing on the picture of the candy .
	manualset3
241814	1	427918	16	NULL	NULL	0	NULL	expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For expression during earlier stages than that driven by the polyhedrin ( polh ) very late promoter , transfer vectors were generated in which this promoter was replaced with a green fluorescent protein ( GFP ) gene controlled by a vp39 late promoter modified to contain HR3 , one of the homologous DNA regions ( HRs ) of Bombyxmori nuclear polyhedrosis virus ( BmNPV ) .
	manualset3
241815	2	427918	16	NULL	NULL	0	NULL	stages	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	For expression during earlier stages than that driven by the polyhedrin ( polh ) very late promoter , transfer vectors were generated in which this promoter was replaced with a green fluorescent protein ( GFP ) gene controlled by a vp39 late promoter modified to contain HR3 , one of the homologous DNA regions ( HRs ) of Bombyxmori nuclear polyhedrosis virus ( BmNPV ) .
	manualset3
241816	3	427918	16	NULL	NULL	0	NULL	polyhedrin ( polh ) very late promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	For expression during earlier stages than that driven by the polyhedrin ( polh ) very late promoter , transfer vectors were generated in which this promoter was replaced with a green fluorescent protein ( GFP ) gene controlled by a vp39 late promoter modified to contain HR3 , one of the homologous DNA regions ( HRs ) of Bombyxmori nuclear polyhedrosis virus ( BmNPV ) .
	manualset3
241817	4	427918	16	NULL	NULL	NULL	NULL	transfer vectors	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For expression during earlier stages than that driven by the polyhedrin ( polh ) very late promoter , transfer vectors were generated in which this promoter was replaced with a green fluorescent protein ( GFP ) gene controlled by a vp39 late promoter modified to contain HR3 , one of the homologous DNA regions ( HRs ) of Bombyxmori nuclear polyhedrosis virus ( BmNPV ) .
	manualset3
241818	5	427918	16	NULL	NULL	0	NULL	promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	For expression during earlier stages than that driven by the polyhedrin ( polh ) very late promoter , transfer vectors were generated in which this promoter was replaced with a green fluorescent protein ( GFP ) gene controlled by a vp39 late promoter modified to contain HR3 , one of the homologous DNA regions ( HRs ) of Bombyxmori nuclear polyhedrosis virus ( BmNPV ) .
	manualset3
241819	6	427918	16	NULL	NULL	0	NULL	green fluorescent protein ( GFP ) gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	For expression during earlier stages than that driven by the polyhedrin ( polh ) very late promoter , transfer vectors were generated in which this promoter was replaced with a green fluorescent protein ( GFP ) gene controlled by a vp39 late promoter modified to contain HR3 , one of the homologous DNA regions ( HRs ) of Bombyxmori nuclear polyhedrosis virus ( BmNPV ) .
	manualset3
241820	7	427918	16	NULL	NULL	0	NULL	vp39 late promoter	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	For expression during earlier stages than that driven by the polyhedrin ( polh ) very late promoter , transfer vectors were generated in which this promoter was replaced with a green fluorescent protein ( GFP ) gene controlled by a vp39 late promoter modified to contain HR3 , one of the homologous DNA regions ( HRs ) of Bombyxmori nuclear polyhedrosis virus ( BmNPV ) .
	manualset3
241821	8	427918	16	NULL	NULL	0	NULL	HR3	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	For expression during earlier stages than that driven by the polyhedrin ( polh ) very late promoter , transfer vectors were generated in which this promoter was replaced with a green fluorescent protein ( GFP ) gene controlled by a vp39 late promoter modified to contain HR3 , one of the homologous DNA regions ( HRs ) of Bombyxmori nuclear polyhedrosis virus ( BmNPV ) .
	manualset3
241822	9	427918	16	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For expression during earlier stages than that driven by the polyhedrin ( polh ) very late promoter , transfer vectors were generated in which this promoter was replaced with a green fluorescent protein ( GFP ) gene controlled by a vp39 late promoter modified to contain HR3 , one of the homologous DNA regions ( HRs ) of Bombyxmori nuclear polyhedrosis virus ( BmNPV ) .
	manualset3
241823	10	427918	16	NULL	NULL	0	NULL	homologous DNA regions ( HRs ) 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	For expression during earlier stages than that driven by the polyhedrin ( polh ) very late promoter , transfer vectors were generated in which this promoter was replaced with a green fluorescent protein ( GFP ) gene controlled by a vp39 late promoter modified to contain HR3 , one of the homologous DNA regions ( HRs ) of Bombyxmori nuclear polyhedrosis virus ( BmNPV ) .
	manualset3
241824	11	427918	16	NULL	NULL	0	NULL	Bombyxmori nuclear polyhedrosis virus ( BmNPV )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For expression during earlier stages than that driven by the polyhedrin ( polh ) very late promoter , transfer vectors were generated in which this promoter was replaced with a green fluorescent protein ( GFP ) gene controlled by a vp39 late promoter modified to contain HR3 , one of the homologous DNA regions ( HRs ) of Bombyxmori nuclear polyhedrosis virus ( BmNPV ) .
	manualset3
241825	1	427919	16	NULL	NULL	0	NULL	fMRI data	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For fMRI data , both conventional analysis with a canonical HRF and an HRF-model-free analysis were performed .
	manualset3
241826	2	427919	16	NULL	NULL	NULL	NULL	conventional analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For fMRI data , both conventional analysis with a canonical HRF and an HRF-model-free analysis were performed .
	manualset3
241827	3	427919	16	NULL	NULL	NULL	NULL	canonical HRF	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For fMRI data , both conventional analysis with a canonical HRF and an HRF-model-free analysis were performed .
	manualset3
241828	4	427919	16	NULL	NULL	NULL	NULL	HRF-model-free analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For fMRI data , both conventional analysis with a canonical HRF and an HRF-model-free analysis were performed .
	manualset3
241829	1	427920	16	NULL	NULL	NULL	NULL	genetic polymorphism	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Relation of genetic polymorphism of NQO1 and GSTT1 with risks of chronic benzene poisoning ) .
	manualset3
241830	2	427920	16	NULL	NULL	0	NULL	NQO1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relation of genetic polymorphism of NQO1 and GSTT1 with risks of chronic benzene poisoning ) .
	manualset3
241831	3	427920	16	NULL	NULL	0	NULL	GSTT1	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relation of genetic polymorphism of NQO1 and GSTT1 with risks of chronic benzene poisoning ) .
	manualset3
241832	4	427920	16	NULL	NULL	0	NULL	risks	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relation of genetic polymorphism of NQO1 and GSTT1 with risks of chronic benzene poisoning ) .
	manualset3
241833	5	427920	16	NULL	NULL	0	NULL	chronic benzene poisoning	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relation of genetic polymorphism of NQO1 and GSTT1 with risks of chronic benzene poisoning ) .
	manualset3
241834	1	427921	16	NULL	NULL	0	NULL	food animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For food animals , both diseased and the healthy populations are studied .
	manualset3
241835	2	427921	16	NULL	NULL	NULL	NULL	diseased populations	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For food animals , both diseased and the healthy populations are studied .
	manualset3
241836	3	427921	16	NULL	NULL	NULL	NULL	healthy populations	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For food animals , both diseased and the healthy populations are studied .
	manualset3
241837	1	427922	16	NULL	NULL	0	NULL	free glycerol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For free glycerol , a linear response was observed from 5 to 70 mg L ( -1 ) with a detection limit of 0.5 mg L ( -1 ) , which corresponds to 2 mg kg ( -1 ) in biodiesel .
	manualset3
241838	2	427922	16	NULL	NULL	0	NULL	linear response	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For free glycerol , a linear response was observed from 5 to 70 mg L ( -1 ) with a detection limit of 0.5 mg L ( -1 ) , which corresponds to 2 mg kg ( -1 ) in biodiesel .
	manualset3
241839	3	427922	16	NULL	NULL	0	NULL	5 to 70 mg L ( -1 )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For free glycerol , a linear response was observed from 5 to 70 mg L ( -1 ) with a detection limit of 0.5 mg L ( -1 ) , which corresponds to 2 mg kg ( -1 ) in biodiesel .
	manualset3
241840	4	427922	16	NULL	NULL	0	NULL	detection limit	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For free glycerol , a linear response was observed from 5 to 70 mg L ( -1 ) with a detection limit of 0.5 mg L ( -1 ) , which corresponds to 2 mg kg ( -1 ) in biodiesel .
	manualset3
241841	5	427922	16	NULL	NULL	0	NULL	0.5 mg L ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For free glycerol , a linear response was observed from 5 to 70 mg L ( -1 ) with a detection limit of 0.5 mg L ( -1 ) , which corresponds to 2 mg kg ( -1 ) in biodiesel .
	manualset3
241842	6	427922	16	NULL	NULL	0	NULL	2 mg kg ( -1 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For free glycerol , a linear response was observed from 5 to 70 mg L ( -1 ) with a detection limit of 0.5 mg L ( -1 ) , which corresponds to 2 mg kg ( -1 ) in biodiesel .
	manualset3
241843	7	427922	16	NULL	NULL	0	NULL	biodiesel	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For free glycerol , a linear response was observed from 5 to 70 mg L ( -1 ) with a detection limit of 0.5 mg L ( -1 ) , which corresponds to 2 mg kg ( -1 ) in biodiesel .
	manualset3
241844	1	427923	16	NULL	NULL	NULL	NULL	medical specialist training	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For full medical specialist training ( up to five years ) the only access requirement should be the equivalent of entrance examinations for French residents .
	manualset3
241845	2	427923	16	NULL	NULL	0	NULL	five years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	For full medical specialist training ( up to five years ) the only access requirement should be the equivalent of entrance examinations for French residents .
	manualset3
241846	3	427923	16	NULL	NULL	0	NULL	access	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For full medical specialist training ( up to five years ) the only access requirement should be the equivalent of entrance examinations for French residents .
	manualset3
241847	4	427923	16	NULL	NULL	NULL	NULL	requirement	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For full medical specialist training ( up to five years ) the only access requirement should be the equivalent of entrance examinations for French residents .
	manualset3
241848	5	427923	16	NULL	NULL	0	NULL	equivalent	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	For full medical specialist training ( up to five years ) the only access requirement should be the equivalent of entrance examinations for French residents .
	manualset3
241849	6	427923	16	NULL	NULL	NULL	NULL	entrance examinations	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For full medical specialist training ( up to five years ) the only access requirement should be the equivalent of entrance examinations for French residents .
	manualset3
241850	7	427923	16	NULL	NULL	0	NULL	French residents	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	For full medical specialist training ( up to five years ) the only access requirement should be the equivalent of entrance examinations for French residents .
	manualset3
241851	1	427924	16	NULL	NULL	NULL	NULL	functional protein lattice	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For generating a functional protein lattice , a chimeric protein was constructed , which comprised the secondary cell wall polymer-binding region and the self-assembly domain of the S-layer protein SbpA from Bacillus sphaericus CCM 2177 , and a single variable region of a heavy chain camel antibody ( cAb-Lys3 ) recognizing lysozyme as antigen .
	manualset3
241852	2	427924	16	NULL	NULL	0	NULL	chimeric protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For generating a functional protein lattice , a chimeric protein was constructed , which comprised the secondary cell wall polymer-binding region and the self-assembly domain of the S-layer protein SbpA from Bacillus sphaericus CCM 2177 , and a single variable region of a heavy chain camel antibody ( cAb-Lys3 ) recognizing lysozyme as antigen .
	manualset3
241853	3	427924	16	NULL	NULL	0	NULL	 secondary cell wall polymer-binding region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	For generating a functional protein lattice , a chimeric protein was constructed , which comprised the secondary cell wall polymer-binding region and the self-assembly domain of the S-layer protein SbpA from Bacillus sphaericus CCM 2177 , and a single variable region of a heavy chain camel antibody ( cAb-Lys3 ) recognizing lysozyme as antigen .
	manualset3
241854	4	427924	16	NULL	NULL	0	NULL	self-assembly domain	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	For generating a functional protein lattice , a chimeric protein was constructed , which comprised the secondary cell wall polymer-binding region and the self-assembly domain of the S-layer protein SbpA from Bacillus sphaericus CCM 2177 , and a single variable region of a heavy chain camel antibody ( cAb-Lys3 ) recognizing lysozyme as antigen .
	manualset3
241855	5	427924	16	NULL	NULL	0	NULL	S-layer protein SbpA	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For generating a functional protein lattice , a chimeric protein was constructed , which comprised the secondary cell wall polymer-binding region and the self-assembly domain of the S-layer protein SbpA from Bacillus sphaericus CCM 2177 , and a single variable region of a heavy chain camel antibody ( cAb-Lys3 ) recognizing lysozyme as antigen .
	manualset3
241856	6	427924	16	NULL	NULL	0	NULL	Bacillus sphaericus CCM 2177	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For generating a functional protein lattice , a chimeric protein was constructed , which comprised the secondary cell wall polymer-binding region and the self-assembly domain of the S-layer protein SbpA from Bacillus sphaericus CCM 2177 , and a single variable region of a heavy chain camel antibody ( cAb-Lys3 ) recognizing lysozyme as antigen .
	manualset3
241857	7	427924	16	NULL	NULL	0	NULL	single variable region	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	For generating a functional protein lattice , a chimeric protein was constructed , which comprised the secondary cell wall polymer-binding region and the self-assembly domain of the S-layer protein SbpA from Bacillus sphaericus CCM 2177 , and a single variable region of a heavy chain camel antibody ( cAb-Lys3 ) recognizing lysozyme as antigen .
	manualset3
241858	8	427924	16	NULL	NULL	NULL	NULL	heavy chain camel antibody ( cAb-Lys3 )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For generating a functional protein lattice , a chimeric protein was constructed , which comprised the secondary cell wall polymer-binding region and the self-assembly domain of the S-layer protein SbpA from Bacillus sphaericus CCM 2177 , and a single variable region of a heavy chain camel antibody ( cAb-Lys3 ) recognizing lysozyme as antigen .
	manualset3
241859	9	427924	16	NULL	NULL	0	NULL	lysozyme	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For generating a functional protein lattice , a chimeric protein was constructed , which comprised the secondary cell wall polymer-binding region and the self-assembly domain of the S-layer protein SbpA from Bacillus sphaericus CCM 2177 , and a single variable region of a heavy chain camel antibody ( cAb-Lys3 ) recognizing lysozyme as antigen .
	manualset3
241860	10	427924	16	NULL	NULL	NULL	NULL	antigen	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For generating a functional protein lattice , a chimeric protein was constructed , which comprised the secondary cell wall polymer-binding region and the self-assembly domain of the S-layer protein SbpA from Bacillus sphaericus CCM 2177 , and a single variable region of a heavy chain camel antibody ( cAb-Lys3 ) recognizing lysozyme as antigen .
	manualset3
241861	1	427925	16	NULL	NULL	NULL	NULL	glass beads	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For glass beads immersed in air or water , we estimate transport mean free paths about half the experimental ones .
	manualset3
241862	2	427925	16	NULL	NULL	0	NULL	air	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For glass beads immersed in air or water , we estimate transport mean free paths about half the experimental ones .
	manualset3
241863	3	427925	16	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For glass beads immersed in air or water , we estimate transport mean free paths about half the experimental ones .
	manualset3
241864	4	427925	16	NULL	NULL	0	NULL	transport mean free paths	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For glass beads immersed in air or water , we estimate transport mean free paths about half the experimental ones .
	manualset3
241866	6	427925	16	NULL	NULL	0	NULL	experimental ones	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For glass beads immersed in air or water , we estimate transport mean free paths about half the experimental ones .
	manualset3
241867	1	427926	16	NULL	NULL	NULL	NULL	Relations	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Relations between the physician and the theater in the Netherlands ) .
	manualset3
241868	2	427926	16	NULL	NULL	0	NULL	physician	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relations between the physician and the theater in the Netherlands ) .
	manualset3
241869	3	427926	16	NULL	NULL	0	NULL	theater	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relations between the physician and the theater in the Netherlands ) .
	manualset3
241870	4	427926	16	NULL	NULL	0	NULL	Netherlands	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relations between the physician and the theater in the Netherlands ) .
	manualset3
241871	1	427927	16	NULL	NULL	0	NULL	in vivo study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For in vivo study , rat pups ( 7 PND , 7 postnatal day ) were injected with AMN082 , L-AP4 or saline before sevoflurane exposure .
	manualset3
241872	2	427927	16	NULL	NULL	0	NULL	rat pups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For in vivo study , rat pups ( 7 PND , 7 postnatal day ) were injected with AMN082 , L-AP4 or saline before sevoflurane exposure .
	manualset3
241873	3	427927	16	NULL	NULL	NULL	NULL	7 PND , 7 postnatal day	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For in vivo study , rat pups ( 7 PND , 7 postnatal day ) were injected with AMN082 , L-AP4 or saline before sevoflurane exposure .
	manualset3
241874	4	427927	16	NULL	NULL	0	NULL	AMN082	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	For in vivo study , rat pups ( 7 PND , 7 postnatal day ) were injected with AMN082 , L-AP4 or saline before sevoflurane exposure .
	manualset3
241875	5	427927	16	NULL	NULL	0	NULL	L-AP4	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	For in vivo study , rat pups ( 7 PND , 7 postnatal day ) were injected with AMN082 , L-AP4 or saline before sevoflurane exposure .
	manualset3
241876	6	427927	16	NULL	NULL	0	NULL	saline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For in vivo study , rat pups ( 7 PND , 7 postnatal day ) were injected with AMN082 , L-AP4 or saline before sevoflurane exposure .
	manualset3
241877	7	427927	16	NULL	NULL	NULL	NULL	sevoflurane exposure	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For in vivo study , rat pups ( 7 PND , 7 postnatal day ) were injected with AMN082 , L-AP4 or saline before sevoflurane exposure .
	manualset3
241879	1	427928	16	NULL	NULL	0	NULL	induction	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For induction by halogenated pyrimidines , a 24-hr incubation of AKR2B cells with caffeine after 5-iodo-2 ' - deoxyuridine treatment resulted in marked suppression of the expression of ecotropic virus .
	manualset3
241880	2	427928	16	NULL	NULL	NULL	NULL	halogenated pyrimidines	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For induction by halogenated pyrimidines , a 24-hr incubation of AKR2B cells with caffeine after 5-iodo-2 ' - deoxyuridine treatment resulted in marked suppression of the expression of ecotropic virus .
	manualset3
241881	3	427928	16	NULL	NULL	0	NULL	24-hr	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	For induction by halogenated pyrimidines , a 24-hr incubation of AKR2B cells with caffeine after 5-iodo-2 ' - deoxyuridine treatment resulted in marked suppression of the expression of ecotropic virus .
	manualset3
241882	4	427928	16	NULL	NULL	0	NULL	incubation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For induction by halogenated pyrimidines , a 24-hr incubation of AKR2B cells with caffeine after 5-iodo-2 ' - deoxyuridine treatment resulted in marked suppression of the expression of ecotropic virus .
	manualset3
241883	5	427928	16	NULL	NULL	0	NULL	AKR2B cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	For induction by halogenated pyrimidines , a 24-hr incubation of AKR2B cells with caffeine after 5-iodo-2 ' - deoxyuridine treatment resulted in marked suppression of the expression of ecotropic virus .
	manualset3
241884	6	427928	16	NULL	NULL	0	NULL	caffeine	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	For induction by halogenated pyrimidines , a 24-hr incubation of AKR2B cells with caffeine after 5-iodo-2 ' - deoxyuridine treatment resulted in marked suppression of the expression of ecotropic virus .
	manualset3
241885	7	427928	16	NULL	NULL	NULL	NULL	5-iodo-2 ' - deoxyuridine treatment	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For induction by halogenated pyrimidines , a 24-hr incubation of AKR2B cells with caffeine after 5-iodo-2 ' - deoxyuridine treatment resulted in marked suppression of the expression of ecotropic virus .
	manualset3
241887	9	427928	16	NULL	NULL	0	NULL	suppression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For induction by halogenated pyrimidines , a 24-hr incubation of AKR2B cells with caffeine after 5-iodo-2 ' - deoxyuridine treatment resulted in marked suppression of the expression of ecotropic virus .
	manualset3
241888	10	427928	16	NULL	NULL	0	NULL	expression	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For induction by halogenated pyrimidines , a 24-hr incubation of AKR2B cells with caffeine after 5-iodo-2 ' - deoxyuridine treatment resulted in marked suppression of the expression of ecotropic virus .
	manualset3
241889	11	427928	16	NULL	NULL	0	NULL	ecotropic virus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For induction by halogenated pyrimidines , a 24-hr incubation of AKR2B cells with caffeine after 5-iodo-2 ' - deoxyuridine treatment resulted in marked suppression of the expression of ecotropic virus .
	manualset3
241892	3	427929	16	NULL	NULL	0	NULL	enzymes	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For instance , changes in enzymes responsible for the biosynthesis of ergosterol , the target of azole activity , lead to azole resistance .
	manualset3
241893	4	427929	16	NULL	NULL	0	NULL	biosynthesis of ergosterol	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For instance , changes in enzymes responsible for the biosynthesis of ergosterol , the target of azole activity , lead to azole resistance .
	manualset3
241894	5	427929	16	NULL	NULL	0	NULL	target	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For instance , changes in enzymes responsible for the biosynthesis of ergosterol , the target of azole activity , lead to azole resistance .
	manualset3
241895	6	427929	16	NULL	NULL	0	NULL	azole activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For instance , changes in enzymes responsible for the biosynthesis of ergosterol , the target of azole activity , lead to azole resistance .
	manualset3
241896	7	427929	16	NULL	NULL	0	NULL	azole resistance	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For instance , changes in enzymes responsible for the biosynthesis of ergosterol , the target of azole activity , lead to azole resistance .
	manualset3
244046	8	427929	16	NULL	NULL	0	NULL	changes	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For instance , changes in enzymes responsible for the biosynthesis of ergosterol , the target of azole activity , lead to azole resistance .
	manualset3
241897	1	427930	16	NULL	NULL	0	NULL	interictal EEG	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For interictal EEG , seizure semiology , ictal EEG , PET and neuropsychology assessment the surgical outcome of patients in whom results were concordant to side of surgery was compared with those discordant or non-lateralising .
	manualset3
241898	2	427930	16	NULL	NULL	0	NULL	seizure semiology	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For interictal EEG , seizure semiology , ictal EEG , PET and neuropsychology assessment the surgical outcome of patients in whom results were concordant to side of surgery was compared with those discordant or non-lateralising .
	manualset3
241899	3	427930	16	NULL	NULL	0	NULL	ictal EEG	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For interictal EEG , seizure semiology , ictal EEG , PET and neuropsychology assessment the surgical outcome of patients in whom results were concordant to side of surgery was compared with those discordant or non-lateralising .
	manualset3
241900	4	427930	16	NULL	NULL	0	NULL	PET	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For interictal EEG , seizure semiology , ictal EEG , PET and neuropsychology assessment the surgical outcome of patients in whom results were concordant to side of surgery was compared with those discordant or non-lateralising .
	manualset3
241901	5	427930	16	NULL	NULL	0	NULL	neuropsychology assessment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For interictal EEG , seizure semiology , ictal EEG , PET and neuropsychology assessment the surgical outcome of patients in whom results were concordant to side of surgery was compared with those discordant or non-lateralising .
	manualset3
241902	6	427930	16	NULL	NULL	0	NULL	surgical outcome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For interictal EEG , seizure semiology , ictal EEG , PET and neuropsychology assessment the surgical outcome of patients in whom results were concordant to side of surgery was compared with those discordant or non-lateralising .
	manualset3
241903	7	427930	16	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	For interictal EEG , seizure semiology , ictal EEG , PET and neuropsychology assessment the surgical outcome of patients in whom results were concordant to side of surgery was compared with those discordant or non-lateralising .
	manualset3
241904	8	427930	16	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For interictal EEG , seizure semiology , ictal EEG , PET and neuropsychology assessment the surgical outcome of patients in whom results were concordant to side of surgery was compared with those discordant or non-lateralising .
	manualset3
241906	10	427930	16	NULL	NULL	0	NULL	surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For interictal EEG , seizure semiology , ictal EEG , PET and neuropsychology assessment the surgical outcome of patients in whom results were concordant to side of surgery was compared with those discordant or non-lateralising .
	manualset3
241907	1	427931	16	NULL	NULL	0	NULL	inulin	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For inulin and APAP-conj , this gradient may be explained by their concentrations within the tubular fluid of the distal nephron .
	manualset3
241908	2	427931	16	NULL	NULL	0	NULL	APAP-conj	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For inulin and APAP-conj , this gradient may be explained by their concentrations within the tubular fluid of the distal nephron .
	manualset3
241909	3	427931	16	NULL	NULL	0	NULL	gradient	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For inulin and APAP-conj , this gradient may be explained by their concentrations within the tubular fluid of the distal nephron .
	manualset3
241910	4	427931	16	NULL	NULL	0	NULL	concentrations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For inulin and APAP-conj , this gradient may be explained by their concentrations within the tubular fluid of the distal nephron .
	manualset3
241911	5	427931	16	NULL	NULL	0	NULL	tubular fluid	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	For inulin and APAP-conj , this gradient may be explained by their concentrations within the tubular fluid of the distal nephron .
	manualset3
241912	6	427931	16	NULL	NULL	0	NULL	distal nephron	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	For inulin and APAP-conj , this gradient may be explained by their concentrations within the tubular fluid of the distal nephron .
	manualset3
241913	1	427932	16	NULL	NULL	0	NULL	irradiation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For irradiation of the prostate + proximal seminal vesicles the unweighted four-field technique provided the best bladder dose sparing .
	manualset3
241914	2	427932	16	NULL	NULL	0	NULL	prostate	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	For irradiation of the prostate + proximal seminal vesicles the unweighted four-field technique provided the best bladder dose sparing .
	manualset3
241915	3	427932	16	NULL	NULL	0	NULL	proximal seminal vesicles	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	For irradiation of the prostate + proximal seminal vesicles the unweighted four-field technique provided the best bladder dose sparing .
	manualset3
241916	4	427932	16	NULL	NULL	0	NULL	unweighted four-field technique	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For irradiation of the prostate + proximal seminal vesicles the unweighted four-field technique provided the best bladder dose sparing .
	manualset3
241917	5	427932	16	NULL	NULL	0	NULL	bladder dose sparing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For irradiation of the prostate + proximal seminal vesicles the unweighted four-field technique provided the best bladder dose sparing .
	manualset3
241918	1	427933	16	NULL	NULL	0	NULL	lateral displacement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For lateral displacement , the restraining force was least at 20 degrees of knee flexion ( 74 N at 10 mm displacement ) , rising to 125 N at 0 degrees and 90 degrees of knee flexion .
	manualset3
241919	2	427933	16	NULL	NULL	0	NULL	restraining force	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For lateral displacement , the restraining force was least at 20 degrees of knee flexion ( 74 N at 10 mm displacement ) , rising to 125 N at 0 degrees and 90 degrees of knee flexion .
	manualset3
241920	3	427933	16	NULL	NULL	0	NULL	20 degrees	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For lateral displacement , the restraining force was least at 20 degrees of knee flexion ( 74 N at 10 mm displacement ) , rising to 125 N at 0 degrees and 90 degrees of knee flexion .
	manualset3
241968	4	427933	16	NULL	NULL	0	NULL	knee flexion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For lateral displacement , the restraining force was least at 20 degrees of knee flexion ( 74 N at 10 mm displacement ) , rising to 125 N at 0 degrees and 90 degrees of knee flexion .
	manualset3
241969	5	427933	16	NULL	NULL	0	NULL	74 N	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For lateral displacement , the restraining force was least at 20 degrees of knee flexion ( 74 N at 10 mm displacement ) , rising to 125 N at 0 degrees and 90 degrees of knee flexion .
	manualset3
241977	6	427933	16	NULL	NULL	0	NULL	10 mm 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For lateral displacement , the restraining force was least at 20 degrees of knee flexion ( 74 N at 10 mm displacement ) , rising to 125 N at 0 degrees and 90 degrees of knee flexion .
	manualset3
241978	7	427933	16	NULL	NULL	0	NULL	displacement	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For lateral displacement , the restraining force was least at 20 degrees of knee flexion ( 74 N at 10 mm displacement ) , rising to 125 N at 0 degrees and 90 degrees of knee flexion .
	manualset3
241984	8	427933	16	NULL	NULL	0	NULL	125 N	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For lateral displacement , the restraining force was least at 20 degrees of knee flexion ( 74 N at 10 mm displacement ) , rising to 125 N at 0 degrees and 90 degrees of knee flexion .
	manualset3
241989	9	427933	16	NULL	NULL	0	NULL	0 degrees	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For lateral displacement , the restraining force was least at 20 degrees of knee flexion ( 74 N at 10 mm displacement ) , rising to 125 N at 0 degrees and 90 degrees of knee flexion .
	manualset3
241991	10	427933	16	NULL	NULL	0	NULL	90 degrees	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For lateral displacement , the restraining force was least at 20 degrees of knee flexion ( 74 N at 10 mm displacement ) , rising to 125 N at 0 degrees and 90 degrees of knee flexion .
	manualset3
241997	11	427933	16	NULL	NULL	0	NULL	knee flexion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For lateral displacement , the restraining force was least at 20 degrees of knee flexion ( 74 N at 10 mm displacement ) , rising to 125 N at 0 degrees and 90 degrees of knee flexion .
	manualset3
242015	1	427934	16	NULL	NULL	0	NULL	Relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relationship between Helicobacter pylori infection and proliferation and apoptosis of gastric epithelial dysplasia cell ) .
	manualset3
242018	2	427934	16	NULL	NULL	0	NULL	Helicobacter pylori infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relationship between Helicobacter pylori infection and proliferation and apoptosis of gastric epithelial dysplasia cell ) .
	manualset3
242590	3	427934	16	NULL	NULL	0	NULL	proliferation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relationship between Helicobacter pylori infection and proliferation and apoptosis of gastric epithelial dysplasia cell ) .
	manualset3
242591	4	427934	16	NULL	NULL	0	NULL	apoptosis	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relationship between Helicobacter pylori infection and proliferation and apoptosis of gastric epithelial dysplasia cell ) .
	manualset3
242592	5	427934	16	NULL	NULL	0	NULL	gastric epithelial dysplasia cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relationship between Helicobacter pylori infection and proliferation and apoptosis of gastric epithelial dysplasia cell ) .
	manualset3
242603	1	427935	16	NULL	NULL	NULL	NULL	maintenance	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For maintenance of anesthesia , halothane was incompatible with the measurement of tcMMEPs .
	manualset3
242604	2	427935	16	NULL	NULL	NULL	NULL	anesthesia	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For maintenance of anesthesia , halothane was incompatible with the measurement of tcMMEPs .
	manualset3
242605	3	427935	16	NULL	NULL	0	NULL	halothane	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	For maintenance of anesthesia , halothane was incompatible with the measurement of tcMMEPs .
	manualset3
242606	4	427935	16	NULL	NULL	0	NULL	measurement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For maintenance of anesthesia , halothane was incompatible with the measurement of tcMMEPs .
	manualset3
242607	5	427935	16	NULL	NULL	0	NULL	tcMMEPs	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For maintenance of anesthesia , halothane was incompatible with the measurement of tcMMEPs .
	manualset3
242611	1	427936	16	NULL	NULL	0	NULL	sufferers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	For many sufferers , a few simple suggestions and proper use of analgesics will provide effective management .
	manualset3
242612	2	427936	16	NULL	NULL	0	NULL	suggestions	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For many sufferers , a few simple suggestions and proper use of analgesics will provide effective management .
	manualset3
242614	3	427936	16	NULL	NULL	NULL	NULL	analgesics	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For many sufferers , a few simple suggestions and proper use of analgesics will provide effective management .
	manualset3
242618	4	427936	16	NULL	NULL	0	NULL	management	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For many sufferers , a few simple suggestions and proper use of analgesics will provide effective management .
	manualset3
242619	1	427937	16	NULL	NULL	0	NULL	years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	For many years , bone scanning has been a valuable tool for the evaluation of bone metastases .
	manualset3
242620	2	427937	16	NULL	NULL	0	NULL	bone scanning	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For many years , bone scanning has been a valuable tool for the evaluation of bone metastases .
	manualset3
242621	3	427937	16	NULL	NULL	0	NULL	tool	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For many years , bone scanning has been a valuable tool for the evaluation of bone metastases .
	manualset3
242622	4	427937	16	NULL	NULL	0	NULL	evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For many years , bone scanning has been a valuable tool for the evaluation of bone metastases .
	manualset3
242623	5	427937	16	NULL	NULL	0	NULL	bone metastases	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For many years , bone scanning has been a valuable tool for the evaluation of bone metastases .
	manualset3
243949	1	427938	16	NULL	NULL	0	NULL	neuroblastoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	For neuroblastoma , a phase I study defined a dose of 13-cis-RA , which was tolerable in patients after myeloablative therapy , and a phase III trial that showed postconsolidation therapy with 13-cis-RA improved EFS for patients with high-risk neuroblastoma .
	manualset3
243950	2	427938	16	NULL	NULL	NULL	NULL	phase I study	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For neuroblastoma , a phase I study defined a dose of 13-cis-RA , which was tolerable in patients after myeloablative therapy , and a phase III trial that showed postconsolidation therapy with 13-cis-RA improved EFS for patients with high-risk neuroblastoma .
	manualset3
243951	3	427938	16	NULL	NULL	0	NULL	dose	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For neuroblastoma , a phase I study defined a dose of 13-cis-RA , which was tolerable in patients after myeloablative therapy , and a phase III trial that showed postconsolidation therapy with 13-cis-RA improved EFS for patients with high-risk neuroblastoma .
	manualset3
243952	4	427938	16	NULL	NULL	0	NULL	13-cis-RA	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	For neuroblastoma , a phase I study defined a dose of 13-cis-RA , which was tolerable in patients after myeloablative therapy , and a phase III trial that showed postconsolidation therapy with 13-cis-RA improved EFS for patients with high-risk neuroblastoma .
	manualset3
243955	5	427938	16	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	For neuroblastoma , a phase I study defined a dose of 13-cis-RA , which was tolerable in patients after myeloablative therapy , and a phase III trial that showed postconsolidation therapy with 13-cis-RA improved EFS for patients with high-risk neuroblastoma .
	manualset3
243956	6	427938	16	NULL	NULL	0	NULL	myeloablative therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For neuroblastoma , a phase I study defined a dose of 13-cis-RA , which was tolerable in patients after myeloablative therapy , and a phase III trial that showed postconsolidation therapy with 13-cis-RA improved EFS for patients with high-risk neuroblastoma .
	manualset3
243957	7	427938	16	NULL	NULL	NULL	NULL	phase III trial	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For neuroblastoma , a phase I study defined a dose of 13-cis-RA , which was tolerable in patients after myeloablative therapy , and a phase III trial that showed postconsolidation therapy with 13-cis-RA improved EFS for patients with high-risk neuroblastoma .
	manualset3
243958	8	427938	16	NULL	NULL	0	NULL	 postconsolidation therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For neuroblastoma , a phase I study defined a dose of 13-cis-RA , which was tolerable in patients after myeloablative therapy , and a phase III trial that showed postconsolidation therapy with 13-cis-RA improved EFS for patients with high-risk neuroblastoma .
	manualset3
243959	9	427938	16	NULL	NULL	0	NULL	13-cis-RA	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	For neuroblastoma , a phase I study defined a dose of 13-cis-RA , which was tolerable in patients after myeloablative therapy , and a phase III trial that showed postconsolidation therapy with 13-cis-RA improved EFS for patients with high-risk neuroblastoma .
	manualset3
244047	10	427938	16	NULL	NULL	0	NULL	EFS	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For neuroblastoma , a phase I study defined a dose of 13-cis-RA , which was tolerable in patients after myeloablative therapy , and a phase III trial that showed postconsolidation therapy with 13-cis-RA improved EFS for patients with high-risk neuroblastoma .
	manualset3
244048	11	427938	16	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	For neuroblastoma , a phase I study defined a dose of 13-cis-RA , which was tolerable in patients after myeloablative therapy , and a phase III trial that showed postconsolidation therapy with 13-cis-RA improved EFS for patients with high-risk neuroblastoma .
	manualset3
244049	12	427938	16	NULL	NULL	0	NULL	high-risk neuroblastoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For neuroblastoma , a phase I study defined a dose of 13-cis-RA , which was tolerable in patients after myeloablative therapy , and a phase III trial that showed postconsolidation therapy with 13-cis-RA improved EFS for patients with high-risk neuroblastoma .
	manualset3
244050	1	427939	16	NULL	NULL	0	NULL	normotensive women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	For normotensive women , results indicate a steady decrease in BP up to 20 weeks of pregnancy , followed by an increase in BP up to the day of delivery , with an average 8 % BP increase between the middle of gestation and delivery .
	manualset3
244051	2	427939	16	NULL	NULL	0	NULL	results	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For normotensive women , results indicate a steady decrease in BP up to 20 weeks of pregnancy , followed by an increase in BP up to the day of delivery , with an average 8 % BP increase between the middle of gestation and delivery .
	manualset3
244052	3	427939	16	NULL	NULL	0	NULL	decrease in BP	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For normotensive women , results indicate a steady decrease in BP up to 20 weeks of pregnancy , followed by an increase in BP up to the day of delivery , with an average 8 % BP increase between the middle of gestation and delivery .
	manualset3
244053	4	427939	16	NULL	NULL	0	NULL	20 weeks	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	For normotensive women , results indicate a steady decrease in BP up to 20 weeks of pregnancy , followed by an increase in BP up to the day of delivery , with an average 8 % BP increase between the middle of gestation and delivery .
	manualset3
244054	5	427939	16	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For normotensive women , results indicate a steady decrease in BP up to 20 weeks of pregnancy , followed by an increase in BP up to the day of delivery , with an average 8 % BP increase between the middle of gestation and delivery .
	manualset3
244055	6	427939	16	NULL	NULL	0	NULL	increase in BP	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For normotensive women , results indicate a steady decrease in BP up to 20 weeks of pregnancy , followed by an increase in BP up to the day of delivery , with an average 8 % BP increase between the middle of gestation and delivery .
	manualset3
244056	7	427939	16	NULL	NULL	0	NULL	day	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	For normotensive women , results indicate a steady decrease in BP up to 20 weeks of pregnancy , followed by an increase in BP up to the day of delivery , with an average 8 % BP increase between the middle of gestation and delivery .
	manualset3
244057	8	427939	16	NULL	NULL	0	NULL	delivery	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For normotensive women , results indicate a steady decrease in BP up to 20 weeks of pregnancy , followed by an increase in BP up to the day of delivery , with an average 8 % BP increase between the middle of gestation and delivery .
	manualset3
244058	9	427939	16	NULL	NULL	0	NULL	average 8 %	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For normotensive women , results indicate a steady decrease in BP up to 20 weeks of pregnancy , followed by an increase in BP up to the day of delivery , with an average 8 % BP increase between the middle of gestation and delivery .
	manualset3
244059	10	427939	16	NULL	NULL	NULL	NULL	BP increase	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For normotensive women , results indicate a steady decrease in BP up to 20 weeks of pregnancy , followed by an increase in BP up to the day of delivery , with an average 8 % BP increase between the middle of gestation and delivery .
	manualset3
244060	11	427939	16	NULL	NULL	NULL	NULL	middle of gestation and delivery	TimePoint												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For normotensive women , results indicate a steady decrease in BP up to 20 weeks of pregnancy , followed by an increase in BP up to the day of delivery , with an average 8 % BP increase between the middle of gestation and delivery .
	manualset3
244062	1	427940	16	NULL	NULL	0	NULL	Acute respiratory distress syndrome	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Acute respiratory distress syndrome as a cause of death in young patients with croupous pneumonia ) .
	manualset3
244063	2	427940	16	NULL	NULL	NULL	NULL	cause of death	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Acute respiratory distress syndrome as a cause of death in young patients with croupous pneumonia ) .
	manualset3
244065	4	427940	16	NULL	NULL	0	NULL	young patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Acute respiratory distress syndrome as a cause of death in young patients with croupous pneumonia ) .
	manualset3
244066	5	427940	16	NULL	NULL	0	NULL	croupous pneumonia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Acute respiratory distress syndrome as a cause of death in young patients with croupous pneumonia ) .
	manualset3
244067	1	427941	16	NULL	NULL	0	NULL	frequency	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relative frequency of esophageal squamous carcinoma and adenocarcinoma in a series of endoscopic biopsies performed in Rosario , Argentina ) .
	manualset3
244068	2	427941	16	NULL	NULL	NULL	NULL	esophageal squamous carcinoma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Relative frequency of esophageal squamous carcinoma and adenocarcinoma in a series of endoscopic biopsies performed in Rosario , Argentina ) .
	manualset3
244069	3	427941	16	NULL	NULL	NULL	NULL	esophageal squamous adenocarcinoma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Relative frequency of esophageal squamous carcinoma and adenocarcinoma in a series of endoscopic biopsies performed in Rosario , Argentina ) .
	manualset3
244070	4	427941	16	NULL	NULL	0	NULL	series	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relative frequency of esophageal squamous carcinoma and adenocarcinoma in a series of endoscopic biopsies performed in Rosario , Argentina ) .
	manualset3
244071	5	427941	16	NULL	NULL	0	NULL	endoscopic biopsies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relative frequency of esophageal squamous carcinoma and adenocarcinoma in a series of endoscopic biopsies performed in Rosario , Argentina ) .
	manualset3
244072	6	427941	16	NULL	NULL	0	NULL	Rosario	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relative frequency of esophageal squamous carcinoma and adenocarcinoma in a series of endoscopic biopsies performed in Rosario , Argentina ) .
	manualset3
244073	7	427941	16	NULL	NULL	0	NULL	Argentina	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relative frequency of esophageal squamous carcinoma and adenocarcinoma in a series of endoscopic biopsies performed in Rosario , Argentina ) .
	manualset3
244074	1	427942	16	NULL	NULL	0	NULL	novices	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	For novices the absolute VSTM performance was better for physically simple than for complex material , whereas for experts the complexity did not matter-Chinese readers memorized Chinese characters ( Experiment 3 ) .
	manualset3
244075	2	427942	16	NULL	NULL	NULL	NULL	VSTM performance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For novices the absolute VSTM performance was better for physically simple than for complex material , whereas for experts the complexity did not matter-Chinese readers memorized Chinese characters ( Experiment 3 ) .
	manualset3
244076	3	427942	16	NULL	NULL	0	NULL	complex material	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For novices the absolute VSTM performance was better for physically simple than for complex material , whereas for experts the complexity did not matter-Chinese readers memorized Chinese characters ( Experiment 3 ) .
	manualset3
244077	4	427942	16	NULL	NULL	0	NULL	experts	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	For novices the absolute VSTM performance was better for physically simple than for complex material , whereas for experts the complexity did not matter-Chinese readers memorized Chinese characters ( Experiment 3 ) .
	manualset3
244078	5	427942	16	NULL	NULL	0	NULL	complexity	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For novices the absolute VSTM performance was better for physically simple than for complex material , whereas for experts the complexity did not matter-Chinese readers memorized Chinese characters ( Experiment 3 ) .
	manualset3
244079	6	427942	16	NULL	NULL	0	NULL	Chinese readers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	For novices the absolute VSTM performance was better for physically simple than for complex material , whereas for experts the complexity did not matter-Chinese readers memorized Chinese characters ( Experiment 3 ) .
	manualset3
244080	7	427942	16	NULL	NULL	0	NULL	Chinese characters	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For novices the absolute VSTM performance was better for physically simple than for complex material , whereas for experts the complexity did not matter-Chinese readers memorized Chinese characters ( Experiment 3 ) .
	manualset3
244081	8	427942	16	NULL	NULL	0	NULL	Experiment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For novices the absolute VSTM performance was better for physically simple than for complex material , whereas for experts the complexity did not matter-Chinese readers memorized Chinese characters ( Experiment 3 ) .
	manualset3
244082	9	427942	16	NULL	NULL	0	NULL	3	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For novices the absolute VSTM performance was better for physically simple than for complex material , whereas for experts the complexity did not matter-Chinese readers memorized Chinese characters ( Experiment 3 ) .
	manualset3
244148	1	427943	16	NULL	NULL	0	NULL	polymorphisms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For one of these polymorphisms ( G58836C in intron 13 ) , the association between AD and the C allele was found to be significant ( odds ratio = 1.73 , 95 % CI : 1.12-2 .67 , P = 0.012 ) .
	manualset3
244149	2	427943	16	NULL	NULL	0	NULL	G58836C in intron 13	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	For one of these polymorphisms ( G58836C in intron 13 ) , the association between AD and the C allele was found to be significant ( odds ratio = 1.73 , 95 % CI : 1.12-2 .67 , P = 0.012 ) .
	manualset3
244150	3	427943	16	NULL	NULL	0	NULL	association	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	For one of these polymorphisms ( G58836C in intron 13 ) , the association between AD and the C allele was found to be significant ( odds ratio = 1.73 , 95 % CI : 1.12-2 .67 , P = 0.012 ) .
	manualset3
244151	4	427943	16	NULL	NULL	0	NULL	AD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	For one of these polymorphisms ( G58836C in intron 13 ) , the association between AD and the C allele was found to be significant ( odds ratio = 1.73 , 95 % CI : 1.12-2 .67 , P = 0.012 ) .
	manualset3
244152	5	427943	16	NULL	NULL	0	NULL	C allele	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For one of these polymorphisms ( G58836C in intron 13 ) , the association between AD and the C allele was found to be significant ( odds ratio = 1.73 , 95 % CI : 1.12-2 .67 , P = 0.012 ) .
	manualset3
244153	6	427943	16	NULL	NULL	0	NULL	odds ratio = 1.73	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For one of these polymorphisms ( G58836C in intron 13 ) , the association between AD and the C allele was found to be significant ( odds ratio = 1.73 , 95 % CI : 1.12-2 .67 , P = 0.012 ) .
	manualset3
244154	7	427943	16	NULL	NULL	0	NULL	95 % CI : 1.12-2 .67	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For one of these polymorphisms ( G58836C in intron 13 ) , the association between AD and the C allele was found to be significant ( odds ratio = 1.73 , 95 % CI : 1.12-2 .67 , P = 0.012 ) .
	manualset3
244155	8	427943	16	NULL	NULL	0	NULL	P = 0.012	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For one of these polymorphisms ( G58836C in intron 13 ) , the association between AD and the C allele was found to be significant ( odds ratio = 1.73 , 95 % CI : 1.12-2 .67 , P = 0.012 ) .
	manualset3
244156	1	427944	16	NULL	NULL	0	NULL	people	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	For people who do not consume alcohol , Itadori tea may be a suitable substitute for red wine .
	manualset3
244157	2	427944	16	NULL	NULL	0	NULL	alcohol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For people who do not consume alcohol , Itadori tea may be a suitable substitute for red wine .
	manualset3
244158	3	427944	16	NULL	NULL	0	NULL	Itadori tea	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	For people who do not consume alcohol , Itadori tea may be a suitable substitute for red wine .
	manualset3
244159	4	427944	16	NULL	NULL	0	NULL	substitute	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For people who do not consume alcohol , Itadori tea may be a suitable substitute for red wine .
	manualset3
244160	5	427944	16	NULL	NULL	0	NULL	red wine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For people who do not consume alcohol , Itadori tea may be a suitable substitute for red wine .
	manualset3
244192	1	427945	16	NULL	NULL	0	NULL	perfusion CT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For perfusion CT , the value added by MSCT is small .
	manualset3
244193	2	427945	16	NULL	NULL	NULL	NULL	value	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For perfusion CT , the value added by MSCT is small .
	manualset3
244194	3	427945	16	NULL	NULL	0	NULL	MSCT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For perfusion CT , the value added by MSCT is small .
	manualset3
244195	1	427946	16	NULL	NULL	0	NULL	phylogenetic analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For phylogenetic analysis , genes for the gC and gD proteins of these viruses were sequenced .
	manualset3
244196	2	427946	16	NULL	NULL	0	NULL	genes	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	For phylogenetic analysis , genes for the gC and gD proteins of these viruses were sequenced .
	manualset3
244197	3	427946	16	NULL	NULL	0	NULL	gC proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For phylogenetic analysis , genes for the gC and gD proteins of these viruses were sequenced .
	manualset3
244198	4	427946	16	NULL	NULL	0	NULL	gD proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For phylogenetic analysis , genes for the gC and gD proteins of these viruses were sequenced .
	manualset3
244199	5	427946	16	NULL	NULL	0	NULL	viruses	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For phylogenetic analysis , genes for the gC and gD proteins of these viruses were sequenced .
	manualset3
244200	1	427947	16	NULL	NULL	0	NULL	planktonic staphylococci	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For planktonic staphylococci , the MIC was 0.625 g/ml .
	manualset3
244201	2	427947	16	NULL	NULL	NULL	NULL	MIC	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For planktonic staphylococci , the MIC was 0.625 g/ml .
	manualset3
244202	3	427947	16	NULL	NULL	0	NULL	0.625 g/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For planktonic staphylococci , the MIC was 0.625 g/ml .
	manualset3
244203	1	427948	16	NULL	NULL	0	NULL	samples	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For pooled samples from all three regions , the mean fertilization rate ( 51 + / - 14 % ) was less tan for spermatozoa from the PC ( P & lt ; 0.05 ) but was not significantly different from spermatozoa from the DC or VD .
	manualset3
244204	2	427948	16	NULL	NULL	0	NULL	three regions	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For pooled samples from all three regions , the mean fertilization rate ( 51 + / - 14 % ) was less tan for spermatozoa from the PC ( P & lt ; 0.05 ) but was not significantly different from spermatozoa from the DC or VD .
	manualset3
244205	3	427948	16	NULL	NULL	NULL	NULL	mean fertilization rate	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For pooled samples from all three regions , the mean fertilization rate ( 51 + / - 14 % ) was less tan for spermatozoa from the PC ( P & lt ; 0.05 ) but was not significantly different from spermatozoa from the DC or VD .
	manualset3
244206	4	427948	16	NULL	NULL	0	NULL	51 + / - 14 %	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For pooled samples from all three regions , the mean fertilization rate ( 51 + / - 14 % ) was less tan for spermatozoa from the PC ( P & lt ; 0.05 ) but was not significantly different from spermatozoa from the DC or VD .
	manualset3
244208	6	427948	16	NULL	NULL	0	NULL	spermatozoa	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	For pooled samples from all three regions , the mean fertilization rate ( 51 + / - 14 % ) was less tan for spermatozoa from the PC ( P & lt ; 0.05 ) but was not significantly different from spermatozoa from the DC or VD .
	manualset3
244209	7	427948	16	NULL	NULL	0	NULL	PC	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For pooled samples from all three regions , the mean fertilization rate ( 51 + / - 14 % ) was less tan for spermatozoa from the PC ( P & lt ; 0.05 ) but was not significantly different from spermatozoa from the DC or VD .
	manualset3
244210	8	427948	16	NULL	NULL	0	NULL	 P & lt ; 0.05	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For pooled samples from all three regions , the mean fertilization rate ( 51 + / - 14 % ) was less tan for spermatozoa from the PC ( P & lt ; 0.05 ) but was not significantly different from spermatozoa from the DC or VD .
	manualset3
244211	9	427948	16	NULL	NULL	0	NULL	spermatozoa	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	For pooled samples from all three regions , the mean fertilization rate ( 51 + / - 14 % ) was less tan for spermatozoa from the PC ( P & lt ; 0.05 ) but was not significantly different from spermatozoa from the DC or VD .
	manualset3
244212	10	427948	16	NULL	NULL	0	NULL	DC	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For pooled samples from all three regions , the mean fertilization rate ( 51 + / - 14 % ) was less tan for spermatozoa from the PC ( P & lt ; 0.05 ) but was not significantly different from spermatozoa from the DC or VD .
	manualset3
244213	11	427948	16	NULL	NULL	0	NULL	VD	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For pooled samples from all three regions , the mean fertilization rate ( 51 + / - 14 % ) was less tan for spermatozoa from the PC ( P & lt ; 0.05 ) but was not significantly different from spermatozoa from the DC or VD .
	manualset3
244218	1	427949	16	NULL	NULL	0	NULL	prisoners	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	For prisoners : mean retinol was 0.840.49 mol/L ; 43.9 % ( 95 % CI 35.9 , 52.2 ) had VAD ( retinol & lt ; 0.70 mol/L ) ; 9.6 % ( 95 % CI 5.1 , 17.0 ) self-reported nyctalopia prior to , and 36.1 % ( 95 % CI 27.7 , 45.5 ) after incarceration ; 10.9 % ( 95 % CI 6.7 , 17.0 ) exhibited at least one sign of xerophthalmia ( 2 had fundus changes ; all 4 with more than conjunctival xerosis alone had severe ( & lt ; 0.35 mol/L ) retinol deficiency ) .
	manualset3
244224	3	427949	16	NULL	NULL	0	NULL	retinol	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	For prisoners : mean retinol was 0.840.49 mol/L ; 43.9 % ( 95 % CI 35.9 , 52.2 ) had VAD ( retinol & lt ; 0.70 mol/L ) ; 9.6 % ( 95 % CI 5.1 , 17.0 ) self-reported nyctalopia prior to , and 36.1 % ( 95 % CI 27.7 , 45.5 ) after incarceration ; 10.9 % ( 95 % CI 6.7 , 17.0 ) exhibited at least one sign of xerophthalmia ( 2 had fundus changes ; all 4 with more than conjunctival xerosis alone had severe ( & lt ; 0.35 mol/L ) retinol deficiency ) .
	manualset3
244227	4	427949	16	NULL	NULL	0	NULL	0.840.49 mol/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For prisoners : mean retinol was 0.840.49 mol/L ; 43.9 % ( 95 % CI 35.9 , 52.2 ) had VAD ( retinol & lt ; 0.70 mol/L ) ; 9.6 % ( 95 % CI 5.1 , 17.0 ) self-reported nyctalopia prior to , and 36.1 % ( 95 % CI 27.7 , 45.5 ) after incarceration ; 10.9 % ( 95 % CI 6.7 , 17.0 ) exhibited at least one sign of xerophthalmia ( 2 had fundus changes ; all 4 with more than conjunctival xerosis alone had severe ( & lt ; 0.35 mol/L ) retinol deficiency ) .
	manualset3
244230	5	427949	16	NULL	NULL	0	NULL	43.9 % ( 95 % CI 35.9 , 52.2 )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For prisoners : mean retinol was 0.840.49 mol/L ; 43.9 % ( 95 % CI 35.9 , 52.2 ) had VAD ( retinol & lt ; 0.70 mol/L ) ; 9.6 % ( 95 % CI 5.1 , 17.0 ) self-reported nyctalopia prior to , and 36.1 % ( 95 % CI 27.7 , 45.5 ) after incarceration ; 10.9 % ( 95 % CI 6.7 , 17.0 ) exhibited at least one sign of xerophthalmia ( 2 had fundus changes ; all 4 with more than conjunctival xerosis alone had severe ( & lt ; 0.35 mol/L ) retinol deficiency ) .
	manualset3
244294	6	427949	16	NULL	NULL	0	NULL	VAD	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For prisoners : mean retinol was 0.840.49 mol/L ; 43.9 % ( 95 % CI 35.9 , 52.2 ) had VAD ( retinol & lt ; 0.70 mol/L ) ; 9.6 % ( 95 % CI 5.1 , 17.0 ) self-reported nyctalopia prior to , and 36.1 % ( 95 % CI 27.7 , 45.5 ) after incarceration ; 10.9 % ( 95 % CI 6.7 , 17.0 ) exhibited at least one sign of xerophthalmia ( 2 had fundus changes ; all 4 with more than conjunctival xerosis alone had severe ( & lt ; 0.35 mol/L ) retinol deficiency ) .
	manualset3
244322	7	427949	16	NULL	NULL	0	NULL	retinol & lt ; 0.70 mol/L	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For prisoners : mean retinol was 0.840.49 mol/L ; 43.9 % ( 95 % CI 35.9 , 52.2 ) had VAD ( retinol & lt ; 0.70 mol/L ) ; 9.6 % ( 95 % CI 5.1 , 17.0 ) self-reported nyctalopia prior to , and 36.1 % ( 95 % CI 27.7 , 45.5 ) after incarceration ; 10.9 % ( 95 % CI 6.7 , 17.0 ) exhibited at least one sign of xerophthalmia ( 2 had fundus changes ; all 4 with more than conjunctival xerosis alone had severe ( & lt ; 0.35 mol/L ) retinol deficiency ) .
	manualset3
244323	8	427949	16	NULL	NULL	0	NULL	9.6 % ( 95 % CI 5.1 , 17.0 )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For prisoners : mean retinol was 0.840.49 mol/L ; 43.9 % ( 95 % CI 35.9 , 52.2 ) had VAD ( retinol & lt ; 0.70 mol/L ) ; 9.6 % ( 95 % CI 5.1 , 17.0 ) self-reported nyctalopia prior to , and 36.1 % ( 95 % CI 27.7 , 45.5 ) after incarceration ; 10.9 % ( 95 % CI 6.7 , 17.0 ) exhibited at least one sign of xerophthalmia ( 2 had fundus changes ; all 4 with more than conjunctival xerosis alone had severe ( & lt ; 0.35 mol/L ) retinol deficiency ) .
	manualset3
244324	9	427949	16	NULL	NULL	0	NULL	nyctalopia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For prisoners : mean retinol was 0.840.49 mol/L ; 43.9 % ( 95 % CI 35.9 , 52.2 ) had VAD ( retinol & lt ; 0.70 mol/L ) ; 9.6 % ( 95 % CI 5.1 , 17.0 ) self-reported nyctalopia prior to , and 36.1 % ( 95 % CI 27.7 , 45.5 ) after incarceration ; 10.9 % ( 95 % CI 6.7 , 17.0 ) exhibited at least one sign of xerophthalmia ( 2 had fundus changes ; all 4 with more than conjunctival xerosis alone had severe ( & lt ; 0.35 mol/L ) retinol deficiency ) .
	manualset3
244325	10	427949	16	NULL	NULL	NULL	NULL	incarceration	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For prisoners : mean retinol was 0.840.49 mol/L ; 43.9 % ( 95 % CI 35.9 , 52.2 ) had VAD ( retinol & lt ; 0.70 mol/L ) ; 9.6 % ( 95 % CI 5.1 , 17.0 ) self-reported nyctalopia prior to , and 36.1 % ( 95 % CI 27.7 , 45.5 ) after incarceration ; 10.9 % ( 95 % CI 6.7 , 17.0 ) exhibited at least one sign of xerophthalmia ( 2 had fundus changes ; all 4 with more than conjunctival xerosis alone had severe ( & lt ; 0.35 mol/L ) retinol deficiency ) .
	manualset3
244326	11	427949	16	NULL	NULL	0	NULL	10.9 % ( 95 % CI 6.7 , 17.0 ) 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For prisoners : mean retinol was 0.840.49 mol/L ; 43.9 % ( 95 % CI 35.9 , 52.2 ) had VAD ( retinol & lt ; 0.70 mol/L ) ; 9.6 % ( 95 % CI 5.1 , 17.0 ) self-reported nyctalopia prior to , and 36.1 % ( 95 % CI 27.7 , 45.5 ) after incarceration ; 10.9 % ( 95 % CI 6.7 , 17.0 ) exhibited at least one sign of xerophthalmia ( 2 had fundus changes ; all 4 with more than conjunctival xerosis alone had severe ( & lt ; 0.35 mol/L ) retinol deficiency ) .
	manualset3
244327	12	427949	16	NULL	NULL	0	NULL	sign	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For prisoners : mean retinol was 0.840.49 mol/L ; 43.9 % ( 95 % CI 35.9 , 52.2 ) had VAD ( retinol & lt ; 0.70 mol/L ) ; 9.6 % ( 95 % CI 5.1 , 17.0 ) self-reported nyctalopia prior to , and 36.1 % ( 95 % CI 27.7 , 45.5 ) after incarceration ; 10.9 % ( 95 % CI 6.7 , 17.0 ) exhibited at least one sign of xerophthalmia ( 2 had fundus changes ; all 4 with more than conjunctival xerosis alone had severe ( & lt ; 0.35 mol/L ) retinol deficiency ) .
	manualset3
244328	13	427949	16	NULL	NULL	0	NULL	xerophthalmia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For prisoners : mean retinol was 0.840.49 mol/L ; 43.9 % ( 95 % CI 35.9 , 52.2 ) had VAD ( retinol & lt ; 0.70 mol/L ) ; 9.6 % ( 95 % CI 5.1 , 17.0 ) self-reported nyctalopia prior to , and 36.1 % ( 95 % CI 27.7 , 45.5 ) after incarceration ; 10.9 % ( 95 % CI 6.7 , 17.0 ) exhibited at least one sign of xerophthalmia ( 2 had fundus changes ; all 4 with more than conjunctival xerosis alone had severe ( & lt ; 0.35 mol/L ) retinol deficiency ) .
	manualset3
244329	14	427949	16	NULL	NULL	0	NULL	2	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For prisoners : mean retinol was 0.840.49 mol/L ; 43.9 % ( 95 % CI 35.9 , 52.2 ) had VAD ( retinol & lt ; 0.70 mol/L ) ; 9.6 % ( 95 % CI 5.1 , 17.0 ) self-reported nyctalopia prior to , and 36.1 % ( 95 % CI 27.7 , 45.5 ) after incarceration ; 10.9 % ( 95 % CI 6.7 , 17.0 ) exhibited at least one sign of xerophthalmia ( 2 had fundus changes ; all 4 with more than conjunctival xerosis alone had severe ( & lt ; 0.35 mol/L ) retinol deficiency ) .
	manualset3
244330	15	427949	16	NULL	NULL	0	NULL	fundus changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For prisoners : mean retinol was 0.840.49 mol/L ; 43.9 % ( 95 % CI 35.9 , 52.2 ) had VAD ( retinol & lt ; 0.70 mol/L ) ; 9.6 % ( 95 % CI 5.1 , 17.0 ) self-reported nyctalopia prior to , and 36.1 % ( 95 % CI 27.7 , 45.5 ) after incarceration ; 10.9 % ( 95 % CI 6.7 , 17.0 ) exhibited at least one sign of xerophthalmia ( 2 had fundus changes ; all 4 with more than conjunctival xerosis alone had severe ( & lt ; 0.35 mol/L ) retinol deficiency ) .
	manualset3
244331	16	427949	16	NULL	NULL	0	NULL	4	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For prisoners : mean retinol was 0.840.49 mol/L ; 43.9 % ( 95 % CI 35.9 , 52.2 ) had VAD ( retinol & lt ; 0.70 mol/L ) ; 9.6 % ( 95 % CI 5.1 , 17.0 ) self-reported nyctalopia prior to , and 36.1 % ( 95 % CI 27.7 , 45.5 ) after incarceration ; 10.9 % ( 95 % CI 6.7 , 17.0 ) exhibited at least one sign of xerophthalmia ( 2 had fundus changes ; all 4 with more than conjunctival xerosis alone had severe ( & lt ; 0.35 mol/L ) retinol deficiency ) .
	manualset3
244332	17	427949	16	NULL	NULL	0	NULL	conjunctival xerosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For prisoners : mean retinol was 0.840.49 mol/L ; 43.9 % ( 95 % CI 35.9 , 52.2 ) had VAD ( retinol & lt ; 0.70 mol/L ) ; 9.6 % ( 95 % CI 5.1 , 17.0 ) self-reported nyctalopia prior to , and 36.1 % ( 95 % CI 27.7 , 45.5 ) after incarceration ; 10.9 % ( 95 % CI 6.7 , 17.0 ) exhibited at least one sign of xerophthalmia ( 2 had fundus changes ; all 4 with more than conjunctival xerosis alone had severe ( & lt ; 0.35 mol/L ) retinol deficiency ) .
	manualset3
244334	19	427949	16	NULL	NULL	0	NULL	& lt ; 0.35 mol/L	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For prisoners : mean retinol was 0.840.49 mol/L ; 43.9 % ( 95 % CI 35.9 , 52.2 ) had VAD ( retinol & lt ; 0.70 mol/L ) ; 9.6 % ( 95 % CI 5.1 , 17.0 ) self-reported nyctalopia prior to , and 36.1 % ( 95 % CI 27.7 , 45.5 ) after incarceration ; 10.9 % ( 95 % CI 6.7 , 17.0 ) exhibited at least one sign of xerophthalmia ( 2 had fundus changes ; all 4 with more than conjunctival xerosis alone had severe ( & lt ; 0.35 mol/L ) retinol deficiency ) .
	manualset3
244335	20	427949	16	NULL	NULL	0	NULL	severe retinol deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For prisoners : mean retinol was 0.840.49 mol/L ; 43.9 % ( 95 % CI 35.9 , 52.2 ) had VAD ( retinol & lt ; 0.70 mol/L ) ; 9.6 % ( 95 % CI 5.1 , 17.0 ) self-reported nyctalopia prior to , and 36.1 % ( 95 % CI 27.7 , 45.5 ) after incarceration ; 10.9 % ( 95 % CI 6.7 , 17.0 ) exhibited at least one sign of xerophthalmia ( 2 had fundus changes ; all 4 with more than conjunctival xerosis alone had severe ( & lt ; 0.35 mol/L ) retinol deficiency ) .
	manualset3
246314	21	427949	16	NULL	NULL	0	NULL	36.1 % ( 95 % CI 27.7 , 45.5 )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For prisoners : mean retinol was 0.840.49 mol/L ; 43.9 % ( 95 % CI 35.9 , 52.2 ) had VAD ( retinol & lt ; 0.70 mol/L ) ; 9.6 % ( 95 % CI 5.1 , 17.0 ) self-reported nyctalopia prior to , and 36.1 % ( 95 % CI 27.7 , 45.5 ) after incarceration ; 10.9 % ( 95 % CI 6.7 , 17.0 ) exhibited at least one sign of xerophthalmia ( 2 had fundus changes ; all 4 with more than conjunctival xerosis alone had severe ( & lt ; 0.35 mol/L ) retinol deficiency ) .
	manualset3
244336	1	427950	16	NULL	NULL	0	NULL	Relief	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relief of dyspnea , right-sided failure and hypoxemia ) .
	manualset3
244675	2	427950	16	NULL	NULL	0	NULL	dyspnea	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relief of dyspnea , right-sided failure and hypoxemia ) .
	manualset3
244676	3	427950	16	NULL	NULL	0	NULL	right-sided failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relief of dyspnea , right-sided failure and hypoxemia ) .
	manualset3
244677	4	427950	16	NULL	NULL	0	NULL	hypoxemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Relief of dyspnea , right-sided failure and hypoxemia ) .
	manualset3
244678	1	427951	16	NULL	NULL	0	NULL	linear alkanes ( C1-nC5 )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For pure linear alkanes ( C1-nC5 ) , the limiting adsorption properties exhibit linear behavior with the alkane carbon number ; the long alkane is preferentially adsorbed over the short alkane at low fugacities , whereas the reverse is found at high fugacities .
	manualset3
244679	2	427951	16	NULL	NULL	NULL	NULL	adsorption properties	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For pure linear alkanes ( C1-nC5 ) , the limiting adsorption properties exhibit linear behavior with the alkane carbon number ; the long alkane is preferentially adsorbed over the short alkane at low fugacities , whereas the reverse is found at high fugacities .
	manualset3
244680	3	427951	16	NULL	NULL	NULL	NULL	linear behavior	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For pure linear alkanes ( C1-nC5 ) , the limiting adsorption properties exhibit linear behavior with the alkane carbon number ; the long alkane is preferentially adsorbed over the short alkane at low fugacities , whereas the reverse is found at high fugacities .
	manualset3
244681	4	427951	16	NULL	NULL	0	NULL	alkane carbon number	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For pure linear alkanes ( C1-nC5 ) , the limiting adsorption properties exhibit linear behavior with the alkane carbon number ; the long alkane is preferentially adsorbed over the short alkane at low fugacities , whereas the reverse is found at high fugacities .
	manualset3
244682	5	427951	16	NULL	NULL	0	NULL	long alkane	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For pure linear alkanes ( C1-nC5 ) , the limiting adsorption properties exhibit linear behavior with the alkane carbon number ; the long alkane is preferentially adsorbed over the short alkane at low fugacities , whereas the reverse is found at high fugacities .
	manualset3
244683	6	427951	16	NULL	NULL	0	NULL	short alkane	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For pure linear alkanes ( C1-nC5 ) , the limiting adsorption properties exhibit linear behavior with the alkane carbon number ; the long alkane is preferentially adsorbed over the short alkane at low fugacities , whereas the reverse is found at high fugacities .
	manualset3
244684	7	427951	16	NULL	NULL	0	NULL	low fugacities	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For pure linear alkanes ( C1-nC5 ) , the limiting adsorption properties exhibit linear behavior with the alkane carbon number ; the long alkane is preferentially adsorbed over the short alkane at low fugacities , whereas the reverse is found at high fugacities .
	manualset3
244685	8	427951	16	NULL	NULL	0	NULL	high fugacities	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For pure linear alkanes ( C1-nC5 ) , the limiting adsorption properties exhibit linear behavior with the alkane carbon number ; the long alkane is preferentially adsorbed over the short alkane at low fugacities , whereas the reverse is found at high fugacities .
	manualset3
244686	1	427952	16	NULL	NULL	NULL	NULL	quantification	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For quantification of clozapine-N-oxide in urine a calibration with diluted calibrators has to be used .
	manualset3
244687	2	427952	16	NULL	NULL	0	NULL	clozapine-N-oxide	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	For quantification of clozapine-N-oxide in urine a calibration with diluted calibrators has to be used .
	manualset3
244688	3	427952	16	NULL	NULL	0	NULL	urine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	For quantification of clozapine-N-oxide in urine a calibration with diluted calibrators has to be used .
	manualset3
244689	4	427952	16	NULL	NULL	0	NULL	calibration	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For quantification of clozapine-N-oxide in urine a calibration with diluted calibrators has to be used .
	manualset3
244690	5	427952	16	NULL	NULL	0	NULL	diluted calibrators	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For quantification of clozapine-N-oxide in urine a calibration with diluted calibrators has to be used .
	manualset3
244691	1	427953	16	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For some rats this beacon unambiguously identified the location of the platform ; for others the beacon was made ambiguous by placement of an identical beacon in a different part of the pool .
	manualset3
244692	2	427953	16	NULL	NULL	0	NULL	beacon	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	For some rats this beacon unambiguously identified the location of the platform ; for others the beacon was made ambiguous by placement of an identical beacon in a different part of the pool .
	manualset3
244693	3	427953	16	NULL	NULL	0	NULL	location	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For some rats this beacon unambiguously identified the location of the platform ; for others the beacon was made ambiguous by placement of an identical beacon in a different part of the pool .
	manualset3
244694	4	427953	16	NULL	NULL	0	NULL	platform	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	For some rats this beacon unambiguously identified the location of the platform ; for others the beacon was made ambiguous by placement of an identical beacon in a different part of the pool .
	manualset3
245195	5	427953	16	NULL	NULL	0	NULL	beacon	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	For some rats this beacon unambiguously identified the location of the platform ; for others the beacon was made ambiguous by placement of an identical beacon in a different part of the pool .
	manualset3
245196	6	427953	16	NULL	NULL	0	NULL	placement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For some rats this beacon unambiguously identified the location of the platform ; for others the beacon was made ambiguous by placement of an identical beacon in a different part of the pool .
	manualset3
245197	7	427953	16	NULL	NULL	0	NULL	beacon	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	For some rats this beacon unambiguously identified the location of the platform ; for others the beacon was made ambiguous by placement of an identical beacon in a different part of the pool .
	manualset3
245198	8	427953	16	NULL	NULL	0	NULL	part	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For some rats this beacon unambiguously identified the location of the platform ; for others the beacon was made ambiguous by placement of an identical beacon in a different part of the pool .
	manualset3
245199	9	427953	16	NULL	NULL	0	NULL	pool	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	For some rats this beacon unambiguously identified the location of the platform ; for others the beacon was made ambiguous by placement of an identical beacon in a different part of the pool .
	manualset3
245200	1	427954	16	NULL	NULL	0	NULL	neurones	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	For some unidentified neurones , 4D7 staining is associated with the presence of acetylcholinesterase indicating that this monoclonal antibody offers a probe for mapping cholinergic neurones in the CNS of Periplaneta americana .
	manualset3
245201	2	427954	16	NULL	NULL	NULL	NULL	4D7	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For some unidentified neurones , 4D7 staining is associated with the presence of acetylcholinesterase indicating that this monoclonal antibody offers a probe for mapping cholinergic neurones in the CNS of Periplaneta americana .
	manualset3
245202	3	427954	16	NULL	NULL	0	NULL	staining	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For some unidentified neurones , 4D7 staining is associated with the presence of acetylcholinesterase indicating that this monoclonal antibody offers a probe for mapping cholinergic neurones in the CNS of Periplaneta americana .
	manualset3
245203	4	427954	16	NULL	NULL	NULL	NULL	presence	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For some unidentified neurones , 4D7 staining is associated with the presence of acetylcholinesterase indicating that this monoclonal antibody offers a probe for mapping cholinergic neurones in the CNS of Periplaneta americana .
	manualset3
245204	5	427954	16	NULL	NULL	0	NULL	acetylcholinesterase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For some unidentified neurones , 4D7 staining is associated with the presence of acetylcholinesterase indicating that this monoclonal antibody offers a probe for mapping cholinergic neurones in the CNS of Periplaneta americana .
	manualset3
245205	6	427954	16	NULL	NULL	NULL	NULL	monoclonal antibody	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For some unidentified neurones , 4D7 staining is associated with the presence of acetylcholinesterase indicating that this monoclonal antibody offers a probe for mapping cholinergic neurones in the CNS of Periplaneta americana .
	manualset3
245206	7	427954	16	NULL	NULL	0	NULL	probe	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	For some unidentified neurones , 4D7 staining is associated with the presence of acetylcholinesterase indicating that this monoclonal antibody offers a probe for mapping cholinergic neurones in the CNS of Periplaneta americana .
	manualset3
245207	8	427954	16	NULL	NULL	0	NULL	mapping	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For some unidentified neurones , 4D7 staining is associated with the presence of acetylcholinesterase indicating that this monoclonal antibody offers a probe for mapping cholinergic neurones in the CNS of Periplaneta americana .
	manualset3
245208	9	427954	16	NULL	NULL	0	NULL	cholinergic neurones	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	For some unidentified neurones , 4D7 staining is associated with the presence of acetylcholinesterase indicating that this monoclonal antibody offers a probe for mapping cholinergic neurones in the CNS of Periplaneta americana .
	manualset3
245209	10	427954	16	NULL	NULL	0	NULL	CNS	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	For some unidentified neurones , 4D7 staining is associated with the presence of acetylcholinesterase indicating that this monoclonal antibody offers a probe for mapping cholinergic neurones in the CNS of Periplaneta americana .
	manualset3
245210	11	427954	16	NULL	NULL	0	NULL	Periplaneta americana	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For some unidentified neurones , 4D7 staining is associated with the presence of acetylcholinesterase indicating that this monoclonal antibody offers a probe for mapping cholinergic neurones in the CNS of Periplaneta americana .
	manualset3
245211	1	427955	16	NULL	NULL	NULL	NULL	sterol concentrations	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For sterol concentrations ranging from 35 to 175 microg mL ( -1 ) , the soxhlet-based extraction process yielded the following recovery efficiencies for coprostanol ( 101 % ) , epicoprostanol ( 97 % ) , cholesterol ( 97 % ) , dihydrocholesterol ( 97 % ) and 5alpha-cholestane ( 111 % ) , whereas the Bligh and Dyer process yielded recoveries of 32 , 41 , 0 , 36 and 51 % , respectively .
	manualset3
245213	3	427955	16	NULL	NULL	0	NULL	35 to 175 microg mL ( -1 )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For sterol concentrations ranging from 35 to 175 microg mL ( -1 ) , the soxhlet-based extraction process yielded the following recovery efficiencies for coprostanol ( 101 % ) , epicoprostanol ( 97 % ) , cholesterol ( 97 % ) , dihydrocholesterol ( 97 % ) and 5alpha-cholestane ( 111 % ) , whereas the Bligh and Dyer process yielded recoveries of 32 , 41 , 0 , 36 and 51 % , respectively .
	manualset3
245214	4	427955	16	NULL	NULL	0	NULL	soxhlet-based extraction process	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For sterol concentrations ranging from 35 to 175 microg mL ( -1 ) , the soxhlet-based extraction process yielded the following recovery efficiencies for coprostanol ( 101 % ) , epicoprostanol ( 97 % ) , cholesterol ( 97 % ) , dihydrocholesterol ( 97 % ) and 5alpha-cholestane ( 111 % ) , whereas the Bligh and Dyer process yielded recoveries of 32 , 41 , 0 , 36 and 51 % , respectively .
	manualset3
245215	5	427955	16	NULL	NULL	0	NULL	recovery efficiencies	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For sterol concentrations ranging from 35 to 175 microg mL ( -1 ) , the soxhlet-based extraction process yielded the following recovery efficiencies for coprostanol ( 101 % ) , epicoprostanol ( 97 % ) , cholesterol ( 97 % ) , dihydrocholesterol ( 97 % ) and 5alpha-cholestane ( 111 % ) , whereas the Bligh and Dyer process yielded recoveries of 32 , 41 , 0 , 36 and 51 % , respectively .
	manualset3
245216	6	427955	16	NULL	NULL	0	NULL	coprostanol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For sterol concentrations ranging from 35 to 175 microg mL ( -1 ) , the soxhlet-based extraction process yielded the following recovery efficiencies for coprostanol ( 101 % ) , epicoprostanol ( 97 % ) , cholesterol ( 97 % ) , dihydrocholesterol ( 97 % ) and 5alpha-cholestane ( 111 % ) , whereas the Bligh and Dyer process yielded recoveries of 32 , 41 , 0 , 36 and 51 % , respectively .
	manualset3
245453	7	427955	16	NULL	NULL	0	NULL	101 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For sterol concentrations ranging from 35 to 175 microg mL ( -1 ) , the soxhlet-based extraction process yielded the following recovery efficiencies for coprostanol ( 101 % ) , epicoprostanol ( 97 % ) , cholesterol ( 97 % ) , dihydrocholesterol ( 97 % ) and 5alpha-cholestane ( 111 % ) , whereas the Bligh and Dyer process yielded recoveries of 32 , 41 , 0 , 36 and 51 % , respectively .
	manualset3
245454	8	427955	16	NULL	NULL	0	NULL	epicoprostanol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For sterol concentrations ranging from 35 to 175 microg mL ( -1 ) , the soxhlet-based extraction process yielded the following recovery efficiencies for coprostanol ( 101 % ) , epicoprostanol ( 97 % ) , cholesterol ( 97 % ) , dihydrocholesterol ( 97 % ) and 5alpha-cholestane ( 111 % ) , whereas the Bligh and Dyer process yielded recoveries of 32 , 41 , 0 , 36 and 51 % , respectively .
	manualset3
245455	9	427955	16	NULL	NULL	NULL	NULL	97 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For sterol concentrations ranging from 35 to 175 microg mL ( -1 ) , the soxhlet-based extraction process yielded the following recovery efficiencies for coprostanol ( 101 % ) , epicoprostanol ( 97 % ) , cholesterol ( 97 % ) , dihydrocholesterol ( 97 % ) and 5alpha-cholestane ( 111 % ) , whereas the Bligh and Dyer process yielded recoveries of 32 , 41 , 0 , 36 and 51 % , respectively .
	manualset3
245456	10	427955	16	NULL	NULL	0	NULL	cholesterol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For sterol concentrations ranging from 35 to 175 microg mL ( -1 ) , the soxhlet-based extraction process yielded the following recovery efficiencies for coprostanol ( 101 % ) , epicoprostanol ( 97 % ) , cholesterol ( 97 % ) , dihydrocholesterol ( 97 % ) and 5alpha-cholestane ( 111 % ) , whereas the Bligh and Dyer process yielded recoveries of 32 , 41 , 0 , 36 and 51 % , respectively .
	manualset3
245457	11	427955	16	NULL	NULL	0	NULL	97 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For sterol concentrations ranging from 35 to 175 microg mL ( -1 ) , the soxhlet-based extraction process yielded the following recovery efficiencies for coprostanol ( 101 % ) , epicoprostanol ( 97 % ) , cholesterol ( 97 % ) , dihydrocholesterol ( 97 % ) and 5alpha-cholestane ( 111 % ) , whereas the Bligh and Dyer process yielded recoveries of 32 , 41 , 0 , 36 and 51 % , respectively .
	manualset3
245458	12	427955	16	NULL	NULL	0	NULL	dihydrocholesterol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For sterol concentrations ranging from 35 to 175 microg mL ( -1 ) , the soxhlet-based extraction process yielded the following recovery efficiencies for coprostanol ( 101 % ) , epicoprostanol ( 97 % ) , cholesterol ( 97 % ) , dihydrocholesterol ( 97 % ) and 5alpha-cholestane ( 111 % ) , whereas the Bligh and Dyer process yielded recoveries of 32 , 41 , 0 , 36 and 51 % , respectively .
	manualset3
245459	13	427955	16	NULL	NULL	0	NULL	97 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For sterol concentrations ranging from 35 to 175 microg mL ( -1 ) , the soxhlet-based extraction process yielded the following recovery efficiencies for coprostanol ( 101 % ) , epicoprostanol ( 97 % ) , cholesterol ( 97 % ) , dihydrocholesterol ( 97 % ) and 5alpha-cholestane ( 111 % ) , whereas the Bligh and Dyer process yielded recoveries of 32 , 41 , 0 , 36 and 51 % , respectively .
	manualset3
245460	14	427955	16	NULL	NULL	0	NULL	5alpha-cholestane	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For sterol concentrations ranging from 35 to 175 microg mL ( -1 ) , the soxhlet-based extraction process yielded the following recovery efficiencies for coprostanol ( 101 % ) , epicoprostanol ( 97 % ) , cholesterol ( 97 % ) , dihydrocholesterol ( 97 % ) and 5alpha-cholestane ( 111 % ) , whereas the Bligh and Dyer process yielded recoveries of 32 , 41 , 0 , 36 and 51 % , respectively .
	manualset3
245461	15	427955	16	NULL	NULL	0	NULL	111 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For sterol concentrations ranging from 35 to 175 microg mL ( -1 ) , the soxhlet-based extraction process yielded the following recovery efficiencies for coprostanol ( 101 % ) , epicoprostanol ( 97 % ) , cholesterol ( 97 % ) , dihydrocholesterol ( 97 % ) and 5alpha-cholestane ( 111 % ) , whereas the Bligh and Dyer process yielded recoveries of 32 , 41 , 0 , 36 and 51 % , respectively .
	manualset3
245462	16	427955	16	NULL	NULL	0	NULL	Bligh and Dyer process	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For sterol concentrations ranging from 35 to 175 microg mL ( -1 ) , the soxhlet-based extraction process yielded the following recovery efficiencies for coprostanol ( 101 % ) , epicoprostanol ( 97 % ) , cholesterol ( 97 % ) , dihydrocholesterol ( 97 % ) and 5alpha-cholestane ( 111 % ) , whereas the Bligh and Dyer process yielded recoveries of 32 , 41 , 0 , 36 and 51 % , respectively .
	manualset3
245463	17	427955	16	NULL	NULL	0	NULL	recoveries	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For sterol concentrations ranging from 35 to 175 microg mL ( -1 ) , the soxhlet-based extraction process yielded the following recovery efficiencies for coprostanol ( 101 % ) , epicoprostanol ( 97 % ) , cholesterol ( 97 % ) , dihydrocholesterol ( 97 % ) and 5alpha-cholestane ( 111 % ) , whereas the Bligh and Dyer process yielded recoveries of 32 , 41 , 0 , 36 and 51 % , respectively .
	manualset3
245464	18	427955	16	NULL	NULL	0	NULL	32 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For sterol concentrations ranging from 35 to 175 microg mL ( -1 ) , the soxhlet-based extraction process yielded the following recovery efficiencies for coprostanol ( 101 % ) , epicoprostanol ( 97 % ) , cholesterol ( 97 % ) , dihydrocholesterol ( 97 % ) and 5alpha-cholestane ( 111 % ) , whereas the Bligh and Dyer process yielded recoveries of 32 , 41 , 0 , 36 and 51 % , respectively .
	manualset3
245465	19	427955	16	NULL	NULL	0	NULL	41 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For sterol concentrations ranging from 35 to 175 microg mL ( -1 ) , the soxhlet-based extraction process yielded the following recovery efficiencies for coprostanol ( 101 % ) , epicoprostanol ( 97 % ) , cholesterol ( 97 % ) , dihydrocholesterol ( 97 % ) and 5alpha-cholestane ( 111 % ) , whereas the Bligh and Dyer process yielded recoveries of 32 , 41 , 0 , 36 and 51 % , respectively .
	manualset3
245466	20	427955	16	NULL	NULL	0	NULL	0 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For sterol concentrations ranging from 35 to 175 microg mL ( -1 ) , the soxhlet-based extraction process yielded the following recovery efficiencies for coprostanol ( 101 % ) , epicoprostanol ( 97 % ) , cholesterol ( 97 % ) , dihydrocholesterol ( 97 % ) and 5alpha-cholestane ( 111 % ) , whereas the Bligh and Dyer process yielded recoveries of 32 , 41 , 0 , 36 and 51 % , respectively .
	manualset3
245467	21	427955	16	NULL	NULL	0	NULL	36 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For sterol concentrations ranging from 35 to 175 microg mL ( -1 ) , the soxhlet-based extraction process yielded the following recovery efficiencies for coprostanol ( 101 % ) , epicoprostanol ( 97 % ) , cholesterol ( 97 % ) , dihydrocholesterol ( 97 % ) and 5alpha-cholestane ( 111 % ) , whereas the Bligh and Dyer process yielded recoveries of 32 , 41 , 0 , 36 and 51 % , respectively .
	manualset3
245468	22	427955	16	NULL	NULL	0	NULL	51 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For sterol concentrations ranging from 35 to 175 microg mL ( -1 ) , the soxhlet-based extraction process yielded the following recovery efficiencies for coprostanol ( 101 % ) , epicoprostanol ( 97 % ) , cholesterol ( 97 % ) , dihydrocholesterol ( 97 % ) and 5alpha-cholestane ( 111 % ) , whereas the Bligh and Dyer process yielded recoveries of 32 , 41 , 0 , 36 and 51 % , respectively .
	manualset3
245217	1	427956	16	NULL	NULL	0	NULL	study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For study of mechanism , the ADAM17 inhibitor TAPI-2 and the PI3K-AKT inhibitor LY294002 were used to counteract high-ADAM17 expression and the activated PI3K-AKT pathway , respectively .
	manualset3
245218	2	427956	16	NULL	NULL	NULL	NULL	mechanism	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For study of mechanism , the ADAM17 inhibitor TAPI-2 and the PI3K-AKT inhibitor LY294002 were used to counteract high-ADAM17 expression and the activated PI3K-AKT pathway , respectively .
	manualset3
245219	3	427956	16	NULL	NULL	NULL	NULL	ADAM17 inhibitor	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For study of mechanism , the ADAM17 inhibitor TAPI-2 and the PI3K-AKT inhibitor LY294002 were used to counteract high-ADAM17 expression and the activated PI3K-AKT pathway , respectively .
	manualset3
245220	4	427956	16	NULL	NULL	0	NULL	TAPI-2	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	For study of mechanism , the ADAM17 inhibitor TAPI-2 and the PI3K-AKT inhibitor LY294002 were used to counteract high-ADAM17 expression and the activated PI3K-AKT pathway , respectively .
	manualset3
245221	5	427956	16	NULL	NULL	NULL	NULL	 PI3K-AKT inhibitor	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For study of mechanism , the ADAM17 inhibitor TAPI-2 and the PI3K-AKT inhibitor LY294002 were used to counteract high-ADAM17 expression and the activated PI3K-AKT pathway , respectively .
	manualset3
245222	6	427956	16	NULL	NULL	0	NULL	LY294002	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	For study of mechanism , the ADAM17 inhibitor TAPI-2 and the PI3K-AKT inhibitor LY294002 were used to counteract high-ADAM17 expression and the activated PI3K-AKT pathway , respectively .
	manualset3
245223	7	427956	16	NULL	NULL	NULL	NULL	ADAM17 expression	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For study of mechanism , the ADAM17 inhibitor TAPI-2 and the PI3K-AKT inhibitor LY294002 were used to counteract high-ADAM17 expression and the activated PI3K-AKT pathway , respectively .
	manualset3
245224	8	427956	16	NULL	NULL	0	NULL	activated PI3K-AKT pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For study of mechanism , the ADAM17 inhibitor TAPI-2 and the PI3K-AKT inhibitor LY294002 were used to counteract high-ADAM17 expression and the activated PI3K-AKT pathway , respectively .
	manualset3
245225	1	427957	16	NULL	NULL	NULL	NULL	action	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Remarkable action of vincaleukoblastine in the treatment of a case of malignant cutaneous reticulosis ) .
	manualset3
245226	2	427957	16	NULL	NULL	0	NULL	vincaleukoblastine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	( Remarkable action of vincaleukoblastine in the treatment of a case of malignant cutaneous reticulosis ) .
	manualset3
245227	3	427957	16	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Remarkable action of vincaleukoblastine in the treatment of a case of malignant cutaneous reticulosis ) .
	manualset3
245228	4	427957	16	NULL	NULL	NULL	NULL	case	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Remarkable action of vincaleukoblastine in the treatment of a case of malignant cutaneous reticulosis ) .
	manualset3
245229	5	427957	16	NULL	NULL	0	NULL	malignant cutaneous reticulosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Remarkable action of vincaleukoblastine in the treatment of a case of malignant cutaneous reticulosis ) .
	manualset3
245230	1	427958	16	NULL	NULL	0	NULL	morphological organization	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For that , we have monitored the morphological organization and spontaneous activity of neuronal networks cultured on multielectrode-arrays during their self-executed evolvement from a mixture of dissociated cells into an active network .
	manualset3
245231	2	427958	16	NULL	NULL	0	NULL	spontaneous activity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For that , we have monitored the morphological organization and spontaneous activity of neuronal networks cultured on multielectrode-arrays during their self-executed evolvement from a mixture of dissociated cells into an active network .
	manualset3
245232	3	427958	16	NULL	NULL	0	NULL	neuronal networks	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	For that , we have monitored the morphological organization and spontaneous activity of neuronal networks cultured on multielectrode-arrays during their self-executed evolvement from a mixture of dissociated cells into an active network .
	manualset3
245233	4	427958	16	NULL	NULL	0	NULL	multielectrode-arrays	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	For that , we have monitored the morphological organization and spontaneous activity of neuronal networks cultured on multielectrode-arrays during their self-executed evolvement from a mixture of dissociated cells into an active network .
	manualset3
245234	5	427958	16	NULL	NULL	0	NULL	evolvement	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For that , we have monitored the morphological organization and spontaneous activity of neuronal networks cultured on multielectrode-arrays during their self-executed evolvement from a mixture of dissociated cells into an active network .
	manualset3
245235	6	427958	16	NULL	NULL	0	NULL	mixture	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For that , we have monitored the morphological organization and spontaneous activity of neuronal networks cultured on multielectrode-arrays during their self-executed evolvement from a mixture of dissociated cells into an active network .
	manualset3
245236	7	427958	16	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	For that , we have monitored the morphological organization and spontaneous activity of neuronal networks cultured on multielectrode-arrays during their self-executed evolvement from a mixture of dissociated cells into an active network .
	manualset3
245237	8	427958	16	NULL	NULL	0	NULL	active network	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For that , we have monitored the morphological organization and spontaneous activity of neuronal networks cultured on multielectrode-arrays during their self-executed evolvement from a mixture of dissociated cells into an active network .
	manualset3
245238	1	427959	16	NULL	NULL	0	NULL	EEG signals	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For that aim , spontaneous EEG signals under different physiological conditions were analyzed .
	manualset3
245239	2	427959	16	NULL	NULL	0	NULL	physiological conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For that aim , spontaneous EEG signals under different physiological conditions were analyzed .
	manualset3
245240	1	427960	16	NULL	NULL	0	NULL	I group	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the I group compared to the NI group , the number of bites by the Anopheles funestus vector per human per night was reduced by 64 % in 1993 and 39 % in 1994 .
	manualset3
245241	2	427960	16	NULL	NULL	0	NULL	NI group	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the I group compared to the NI group , the number of bites by the Anopheles funestus vector per human per night was reduced by 64 % in 1993 and 39 % in 1994 .
	manualset3
245242	3	427960	16	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the I group compared to the NI group , the number of bites by the Anopheles funestus vector per human per night was reduced by 64 % in 1993 and 39 % in 1994 .
	manualset3
245243	4	427960	16	NULL	NULL	0	NULL	bites	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For the I group compared to the NI group , the number of bites by the Anopheles funestus vector per human per night was reduced by 64 % in 1993 and 39 % in 1994 .
	manualset3
245244	5	427960	16	NULL	NULL	0	NULL	Anopheles funestus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For the I group compared to the NI group , the number of bites by the Anopheles funestus vector per human per night was reduced by 64 % in 1993 and 39 % in 1994 .
	manualset3
245245	6	427960	16	NULL	NULL	0	NULL	vector	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For the I group compared to the NI group , the number of bites by the Anopheles funestus vector per human per night was reduced by 64 % in 1993 and 39 % in 1994 .
	manualset3
245246	7	427960	16	NULL	NULL	0	NULL	human	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	For the I group compared to the NI group , the number of bites by the Anopheles funestus vector per human per night was reduced by 64 % in 1993 and 39 % in 1994 .
	manualset3
245247	8	427960	16	NULL	NULL	NULL	NULL	night	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For the I group compared to the NI group , the number of bites by the Anopheles funestus vector per human per night was reduced by 64 % in 1993 and 39 % in 1994 .
	manualset3
245248	9	427960	16	NULL	NULL	0	NULL	64 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the I group compared to the NI group , the number of bites by the Anopheles funestus vector per human per night was reduced by 64 % in 1993 and 39 % in 1994 .
	manualset3
245249	10	427960	16	NULL	NULL	0	NULL	1993	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	For the I group compared to the NI group , the number of bites by the Anopheles funestus vector per human per night was reduced by 64 % in 1993 and 39 % in 1994 .
	manualset3
245250	11	427960	16	NULL	NULL	0	NULL	39 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the I group compared to the NI group , the number of bites by the Anopheles funestus vector per human per night was reduced by 64 % in 1993 and 39 % in 1994 .
	manualset3
245251	12	427960	16	NULL	NULL	0	NULL	1994	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	For the I group compared to the NI group , the number of bites by the Anopheles funestus vector per human per night was reduced by 64 % in 1993 and 39 % in 1994 .
	manualset3
245253	2	427961	16	NULL	NULL	NULL	NULL	OA group	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For the OA group , the Moleca reduced KAM even more as compared to the barefoot condition during midstance .
	manualset3
245254	3	427961	16	NULL	NULL	0	NULL	Moleca	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	For the OA group , the Moleca reduced KAM even more as compared to the barefoot condition during midstance .
	manualset3
245255	4	427961	16	NULL	NULL	0	NULL	KAM	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For the OA group , the Moleca reduced KAM even more as compared to the barefoot condition during midstance .
	manualset3
245256	5	427961	16	NULL	NULL	0	NULL	barefoot condition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For the OA group , the Moleca reduced KAM even more as compared to the barefoot condition during midstance .
	manualset3
245257	6	427961	16	NULL	NULL	0	NULL	midstance	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the OA group , the Moleca reduced KAM even more as compared to the barefoot condition during midstance .
	manualset3
245259	2	427962	16	NULL	NULL	0	NULL	in-frame deletion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For the PDGFRalpha , we observed an in-frame deletion of codons 554 and 555 in a case which also showed a strong immunopositivity for the phosphorylated form of PDGFRalpha .
	manualset3
245260	3	427962	16	NULL	NULL	0	NULL	codons 554	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	For the PDGFRalpha , we observed an in-frame deletion of codons 554 and 555 in a case which also showed a strong immunopositivity for the phosphorylated form of PDGFRalpha .
	manualset3
245261	4	427962	16	NULL	NULL	0	NULL	codons 555	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	For the PDGFRalpha , we observed an in-frame deletion of codons 554 and 555 in a case which also showed a strong immunopositivity for the phosphorylated form of PDGFRalpha .
	manualset3
245262	5	427962	16	NULL	NULL	0	NULL	case	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the PDGFRalpha , we observed an in-frame deletion of codons 554 and 555 in a case which also showed a strong immunopositivity for the phosphorylated form of PDGFRalpha .
	manualset3
245263	6	427962	16	NULL	NULL	0	NULL	immunopositivity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For the PDGFRalpha , we observed an in-frame deletion of codons 554 and 555 in a case which also showed a strong immunopositivity for the phosphorylated form of PDGFRalpha .
	manualset3
245264	7	427962	16	NULL	NULL	NULL	NULL	phosphorylated form of PDGFRalpha	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For the PDGFRalpha , we observed an in-frame deletion of codons 554 and 555 in a case which also showed a strong immunopositivity for the phosphorylated form of PDGFRalpha .
	manualset3
245265	8	427962	16	NULL	NULL	0	NULL	PDGFRalpha	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For the PDGFRalpha , we observed an in-frame deletion of codons 554 and 555 in a case which also showed a strong immunopositivity for the phosphorylated form of PDGFRalpha .
	manualset3
245266	1	427963	16	NULL	NULL	0	NULL	fly	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For the `` selective '' fly Phlebotomus papatasi PpapJ , side chain galactosyl-modifications ( scGal ) of PG repeats play key roles in parasite binding .
	manualset3
245267	2	427963	16	NULL	NULL	0	NULL	Phlebotomus papatasi PpapJ	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For the `` selective '' fly Phlebotomus papatasi PpapJ , side chain galactosyl-modifications ( scGal ) of PG repeats play key roles in parasite binding .
	manualset3
245268	3	427963	16	NULL	NULL	0	NULL	side chain galactosyl-modifications ( scGal )	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For the `` selective '' fly Phlebotomus papatasi PpapJ , side chain galactosyl-modifications ( scGal ) of PG repeats play key roles in parasite binding .
	manualset3
245269	4	427963	16	NULL	NULL	0	NULL	PG repeats	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	For the `` selective '' fly Phlebotomus papatasi PpapJ , side chain galactosyl-modifications ( scGal ) of PG repeats play key roles in parasite binding .
	manualset3
245271	6	427963	16	NULL	NULL	0	NULL	parasite binding	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For the `` selective '' fly Phlebotomus papatasi PpapJ , side chain galactosyl-modifications ( scGal ) of PG repeats play key roles in parasite binding .
	manualset3
245272	1	427964	16	NULL	NULL	0	NULL	antigenotoxicity assays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the antigenotoxicity assays , the different doses of artepillin C were administered simultaneously to doxorubicin ( DXR ; micronucleus test ; 15mgkg ( -1 ) b.w. ) and to methyl methanesulfonate ( MMS ; comet assay ; 40mgkg ( -1 ) b.w. ) .
	manualset3
245273	2	427964	16	NULL	NULL	0	NULL	doses	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the antigenotoxicity assays , the different doses of artepillin C were administered simultaneously to doxorubicin ( DXR ; micronucleus test ; 15mgkg ( -1 ) b.w. ) and to methyl methanesulfonate ( MMS ; comet assay ; 40mgkg ( -1 ) b.w. ) .
	manualset3
245274	3	427964	16	NULL	NULL	0	NULL	artepillin C	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For the antigenotoxicity assays , the different doses of artepillin C were administered simultaneously to doxorubicin ( DXR ; micronucleus test ; 15mgkg ( -1 ) b.w. ) and to methyl methanesulfonate ( MMS ; comet assay ; 40mgkg ( -1 ) b.w. ) .
	manualset3
245275	4	427964	16	NULL	NULL	0	NULL	doxorubicin ( DXR	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	For the antigenotoxicity assays , the different doses of artepillin C were administered simultaneously to doxorubicin ( DXR ; micronucleus test ; 15mgkg ( -1 ) b.w. ) and to methyl methanesulfonate ( MMS ; comet assay ; 40mgkg ( -1 ) b.w. ) .
	manualset3
245276	5	427964	16	NULL	NULL	0	NULL	micronucleus test	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the antigenotoxicity assays , the different doses of artepillin C were administered simultaneously to doxorubicin ( DXR ; micronucleus test ; 15mgkg ( -1 ) b.w. ) and to methyl methanesulfonate ( MMS ; comet assay ; 40mgkg ( -1 ) b.w. ) .
	manualset3
245277	6	427964	16	NULL	NULL	NULL	NULL	15mgkg ( -1 ) b.w. 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For the antigenotoxicity assays , the different doses of artepillin C were administered simultaneously to doxorubicin ( DXR ; micronucleus test ; 15mgkg ( -1 ) b.w. ) and to methyl methanesulfonate ( MMS ; comet assay ; 40mgkg ( -1 ) b.w. ) .
	manualset3
245278	7	427964	16	NULL	NULL	0	NULL	methyl methanesulfonate ( MMS 	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	For the antigenotoxicity assays , the different doses of artepillin C were administered simultaneously to doxorubicin ( DXR ; micronucleus test ; 15mgkg ( -1 ) b.w. ) and to methyl methanesulfonate ( MMS ; comet assay ; 40mgkg ( -1 ) b.w. ) .
	manualset3
245279	8	427964	16	NULL	NULL	0	NULL	comet assay	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the antigenotoxicity assays , the different doses of artepillin C were administered simultaneously to doxorubicin ( DXR ; micronucleus test ; 15mgkg ( -1 ) b.w. ) and to methyl methanesulfonate ( MMS ; comet assay ; 40mgkg ( -1 ) b.w. ) .
	manualset3
245280	9	427964	16	NULL	NULL	NULL	NULL	40mgkg ( -1 ) b.w	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For the antigenotoxicity assays , the different doses of artepillin C were administered simultaneously to doxorubicin ( DXR ; micronucleus test ; 15mgkg ( -1 ) b.w. ) and to methyl methanesulfonate ( MMS ; comet assay ; 40mgkg ( -1 ) b.w. ) .
	manualset3
245282	2	427965	16	NULL	NULL	0	NULL	predictor variable	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	For the case of a single predictor or explanatory ( independent ) variable , X , a plot can be generated with X represented by the abscissa ( i.e. , horizontal axis ) and P ( Y-1 / X ) represented by the ordinate ( i.e. , vertical axis ) .
	manualset3
245283	3	427965	16	NULL	NULL	0	NULL	 explanatory ( independent ) variable	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	For the case of a single predictor or explanatory ( independent ) variable , X , a plot can be generated with X represented by the abscissa ( i.e. , horizontal axis ) and P ( Y-1 / X ) represented by the ordinate ( i.e. , vertical axis ) .
	manualset3
245284	4	427965	16	NULL	NULL	0	NULL	X	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the case of a single predictor or explanatory ( independent ) variable , X , a plot can be generated with X represented by the abscissa ( i.e. , horizontal axis ) and P ( Y-1 / X ) represented by the ordinate ( i.e. , vertical axis ) .
	manualset3
245285	5	427965	16	NULL	NULL	NULL	NULL	plot	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For the case of a single predictor or explanatory ( independent ) variable , X , a plot can be generated with X represented by the abscissa ( i.e. , horizontal axis ) and P ( Y-1 / X ) represented by the ordinate ( i.e. , vertical axis ) .
	manualset3
245286	6	427965	16	NULL	NULL	0	NULL	X	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the case of a single predictor or explanatory ( independent ) variable , X , a plot can be generated with X represented by the abscissa ( i.e. , horizontal axis ) and P ( Y-1 / X ) represented by the ordinate ( i.e. , vertical axis ) .
	manualset3
245287	7	427965	16	NULL	NULL	0	NULL	abscissa	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the case of a single predictor or explanatory ( independent ) variable , X , a plot can be generated with X represented by the abscissa ( i.e. , horizontal axis ) and P ( Y-1 / X ) represented by the ordinate ( i.e. , vertical axis ) .
	manualset3
245288	8	427965	16	NULL	NULL	0	NULL	horizontal axis	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the case of a single predictor or explanatory ( independent ) variable , X , a plot can be generated with X represented by the abscissa ( i.e. , horizontal axis ) and P ( Y-1 / X ) represented by the ordinate ( i.e. , vertical axis ) .
	manualset3
245289	9	427965	16	NULL	NULL	0	NULL	P ( Y-1 / X )	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the case of a single predictor or explanatory ( independent ) variable , X , a plot can be generated with X represented by the abscissa ( i.e. , horizontal axis ) and P ( Y-1 / X ) represented by the ordinate ( i.e. , vertical axis ) .
	manualset3
245290	10	427965	16	NULL	NULL	0	NULL	ordinate	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the case of a single predictor or explanatory ( independent ) variable , X , a plot can be generated with X represented by the abscissa ( i.e. , horizontal axis ) and P ( Y-1 / X ) represented by the ordinate ( i.e. , vertical axis ) .
	manualset3
245291	11	427965	16	NULL	NULL	0	NULL	vertical axis	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the case of a single predictor or explanatory ( independent ) variable , X , a plot can be generated with X represented by the abscissa ( i.e. , horizontal axis ) and P ( Y-1 / X ) represented by the ordinate ( i.e. , vertical axis ) .
	manualset3
245270	5	427966	16	NULL	NULL	NULL	NULL	case	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For the case of zero self-propulsion , it is simplified to the equation of motion for infinitesimal fluid particles .
	manualset3
245292	1	427966	16	NULL	NULL	NULL	NULL	self-propulsion	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For the case of zero self-propulsion , it is simplified to the equation of motion for infinitesimal fluid particles .
	manualset3
245293	2	427966	16	NULL	NULL	0	NULL	equation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For the case of zero self-propulsion , it is simplified to the equation of motion for infinitesimal fluid particles .
	manualset3
245294	3	427966	16	NULL	NULL	0	NULL	motion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For the case of zero self-propulsion , it is simplified to the equation of motion for infinitesimal fluid particles .
	manualset3
245295	4	427966	16	NULL	NULL	NULL	NULL	infinitesimal fluid particles	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For the case of zero self-propulsion , it is simplified to the equation of motion for infinitesimal fluid particles .
	manualset3
245296	1	427967	16	NULL	NULL	NULL	NULL	result	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Remarkable result of an adrenal medullosclerosis in the course of malignant arterial hypertension ) .
	manualset3
245297	2	427967	16	NULL	NULL	0	NULL	adrenal medullosclerosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Remarkable result of an adrenal medullosclerosis in the course of malignant arterial hypertension ) .
	manualset3
245298	3	427967	16	NULL	NULL	0	NULL	course	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Remarkable result of an adrenal medullosclerosis in the course of malignant arterial hypertension ) .
	manualset3
245299	4	427967	16	NULL	NULL	0	NULL	malignant arterial hypertension	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Remarkable result of an adrenal medullosclerosis in the course of malignant arterial hypertension ) .
	manualset3
245300	1	427968	16	NULL	NULL	0	NULL	classification	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the classification of the analyzed points of the porcelain cards principal component analysis ( PCA ) was used .
	manualset3
245301	2	427968	16	NULL	NULL	0	NULL	analyzed points	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the classification of the analyzed points of the porcelain cards principal component analysis ( PCA ) was used .
	manualset3
245302	3	427968	16	NULL	NULL	0	NULL	porcelain cards	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	For the classification of the analyzed points of the porcelain cards principal component analysis ( PCA ) was used .
	manualset3
245303	4	427968	16	NULL	NULL	0	NULL	principal component analysis ( PCA )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the classification of the analyzed points of the porcelain cards principal component analysis ( PCA ) was used .
	manualset3
245304	1	427969	16	NULL	NULL	0	NULL	factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the different factors under consideration , especially plasma protein binding , the weight and the age of the patient plays an important role .
	manualset3
245305	2	427969	16	NULL	NULL	0	NULL	consideration	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For the different factors under consideration , especially plasma protein binding , the weight and the age of the patient plays an important role .
	manualset3
245306	3	427969	16	NULL	NULL	0	NULL	plasma protein binding	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For the different factors under consideration , especially plasma protein binding , the weight and the age of the patient plays an important role .
	manualset3
245307	4	427969	16	NULL	NULL	0	NULL	weight	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the different factors under consideration , especially plasma protein binding , the weight and the age of the patient plays an important role .
	manualset3
245308	5	427969	16	NULL	NULL	0	NULL	age	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For the different factors under consideration , especially plasma protein binding , the weight and the age of the patient plays an important role .
	manualset3
245309	6	427969	16	NULL	NULL	0	NULL	patient	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	For the different factors under consideration , especially plasma protein binding , the weight and the age of the patient plays an important role .
	manualset3
245310	7	427969	16	NULL	NULL	NULL	NULL	role	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For the different factors under consideration , especially plasma protein binding , the weight and the age of the patient plays an important role .
	manualset3
245311	1	427970	16	NULL	NULL	0	NULL	evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the evaluation of the role of MAPKs , PD98059 , SB202190 and SP600125 were used as MAPK inhibitors for ERK-1 / 2 , p38 and JNK .
	manualset3
245312	2	427970	16	NULL	NULL	NULL	NULL	role	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For the evaluation of the role of MAPKs , PD98059 , SB202190 and SP600125 were used as MAPK inhibitors for ERK-1 / 2 , p38 and JNK .
	manualset3
245313	3	427970	16	NULL	NULL	NULL	NULL	MAPKs	GeneOrProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For the evaluation of the role of MAPKs , PD98059 , SB202190 and SP600125 were used as MAPK inhibitors for ERK-1 / 2 , p38 and JNK .
	manualset3
245314	4	427970	16	NULL	NULL	0	NULL	PD98059	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	For the evaluation of the role of MAPKs , PD98059 , SB202190 and SP600125 were used as MAPK inhibitors for ERK-1 / 2 , p38 and JNK .
	manualset3
245315	5	427970	16	NULL	NULL	0	NULL	SB202190	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	For the evaluation of the role of MAPKs , PD98059 , SB202190 and SP600125 were used as MAPK inhibitors for ERK-1 / 2 , p38 and JNK .
	manualset3
245316	6	427970	16	NULL	NULL	0	NULL	SP600125	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	For the evaluation of the role of MAPKs , PD98059 , SB202190 and SP600125 were used as MAPK inhibitors for ERK-1 / 2 , p38 and JNK .
	manualset3
245317	7	427970	16	NULL	NULL	0	NULL	MAPK inhibitors	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For the evaluation of the role of MAPKs , PD98059 , SB202190 and SP600125 were used as MAPK inhibitors for ERK-1 / 2 , p38 and JNK .
	manualset3
245318	8	427970	16	NULL	NULL	0	NULL	ERK-1 / 2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For the evaluation of the role of MAPKs , PD98059 , SB202190 and SP600125 were used as MAPK inhibitors for ERK-1 / 2 , p38 and JNK .
	manualset3
245319	9	427970	16	NULL	NULL	0	NULL	p38	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For the evaluation of the role of MAPKs , PD98059 , SB202190 and SP600125 were used as MAPK inhibitors for ERK-1 / 2 , p38 and JNK .
	manualset3
245320	10	427970	16	NULL	NULL	0	NULL	JNK	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For the evaluation of the role of MAPKs , PD98059 , SB202190 and SP600125 were used as MAPK inhibitors for ERK-1 / 2 , p38 and JNK .
	manualset3
245321	1	427971	16	NULL	NULL	0	NULL	skin construct	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	For the first time in a skin construct , the expression of prolyl-4-hydroxylase was detected in dermal fibroblasts by in situ hybridization .
	manualset3
245322	2	427971	16	NULL	NULL	NULL	NULL	expression of prolyl-4-hydroxylase	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For the first time in a skin construct , the expression of prolyl-4-hydroxylase was detected in dermal fibroblasts by in situ hybridization .
	manualset3
245324	4	427971	16	NULL	NULL	0	NULL	dermal fibroblasts	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	For the first time in a skin construct , the expression of prolyl-4-hydroxylase was detected in dermal fibroblasts by in situ hybridization .
	manualset3
245325	5	427971	16	NULL	NULL	0	NULL	in situ hybridization	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the first time in a skin construct , the expression of prolyl-4-hydroxylase was detected in dermal fibroblasts by in situ hybridization .
	manualset3
245326	1	427972	16	NULL	NULL	0	NULL	fraction	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the fraction of the analog that could be substituted , the dissociation constants for MgATP and ATP were estimated to be 0.27 + / - 0.09 and 0.33 + / - 0.15 mM respectively , close to the values determined by equilibrium dialysis .
	manualset3
245327	2	427972	16	NULL	NULL	0	NULL	analog	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For the fraction of the analog that could be substituted , the dissociation constants for MgATP and ATP were estimated to be 0.27 + / - 0.09 and 0.33 + / - 0.15 mM respectively , close to the values determined by equilibrium dialysis .
	manualset3
245328	3	427972	16	NULL	NULL	NULL	NULL	dissociation constants	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For the fraction of the analog that could be substituted , the dissociation constants for MgATP and ATP were estimated to be 0.27 + / - 0.09 and 0.33 + / - 0.15 mM respectively , close to the values determined by equilibrium dialysis .
	manualset3
245329	4	427972	16	NULL	NULL	0	NULL	MgATP	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For the fraction of the analog that could be substituted , the dissociation constants for MgATP and ATP were estimated to be 0.27 + / - 0.09 and 0.33 + / - 0.15 mM respectively , close to the values determined by equilibrium dialysis .
	manualset3
245330	5	427972	16	NULL	NULL	0	NULL	ATP	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For the fraction of the analog that could be substituted , the dissociation constants for MgATP and ATP were estimated to be 0.27 + / - 0.09 and 0.33 + / - 0.15 mM respectively , close to the values determined by equilibrium dialysis .
	manualset3
245331	6	427972	16	NULL	NULL	0	NULL	0.27 + / - 0.09mM	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the fraction of the analog that could be substituted , the dissociation constants for MgATP and ATP were estimated to be 0.27 + / - 0.09 and 0.33 + / - 0.15 mM respectively , close to the values determined by equilibrium dialysis .
	manualset3
245332	7	427972	16	NULL	NULL	0	NULL	0.33 + / - 0.15 mM	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the fraction of the analog that could be substituted , the dissociation constants for MgATP and ATP were estimated to be 0.27 + / - 0.09 and 0.33 + / - 0.15 mM respectively , close to the values determined by equilibrium dialysis .
	manualset3
245333	8	427972	16	NULL	NULL	0	NULL	values	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the fraction of the analog that could be substituted , the dissociation constants for MgATP and ATP were estimated to be 0.27 + / - 0.09 and 0.33 + / - 0.15 mM respectively , close to the values determined by equilibrium dialysis .
	manualset3
245334	9	427972	16	NULL	NULL	0	NULL	equilibrium dialysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the fraction of the analog that could be substituted , the dissociation constants for MgATP and ATP were estimated to be 0.27 + / - 0.09 and 0.33 + / - 0.15 mM respectively , close to the values determined by equilibrium dialysis .
	manualset3
245335	1	427973	16	NULL	NULL	NULL	NULL	healthcare industry	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For the healthcare industry , mobile applications provide a new frontier in offering better care and services to patients , and a more flexible and mobile way of communicating with suppliers and patients .
	manualset3
245336	2	427973	16	NULL	NULL	0	NULL	mobile applications	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	For the healthcare industry , mobile applications provide a new frontier in offering better care and services to patients , and a more flexible and mobile way of communicating with suppliers and patients .
	manualset3
245337	3	427973	16	NULL	NULL	0	NULL	frontier	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the healthcare industry , mobile applications provide a new frontier in offering better care and services to patients , and a more flexible and mobile way of communicating with suppliers and patients .
	manualset3
245338	4	427973	16	NULL	NULL	0	NULL	care	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For the healthcare industry , mobile applications provide a new frontier in offering better care and services to patients , and a more flexible and mobile way of communicating with suppliers and patients .
	manualset3
245339	5	427973	16	NULL	NULL	0	NULL	services	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	For the healthcare industry , mobile applications provide a new frontier in offering better care and services to patients , and a more flexible and mobile way of communicating with suppliers and patients .
	manualset3
245340	6	427973	16	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	For the healthcare industry , mobile applications provide a new frontier in offering better care and services to patients , and a more flexible and mobile way of communicating with suppliers and patients .
	manualset3
245341	7	427973	16	NULL	NULL	NULL	NULL	way	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For the healthcare industry , mobile applications provide a new frontier in offering better care and services to patients , and a more flexible and mobile way of communicating with suppliers and patients .
	manualset3
245342	8	427973	16	NULL	NULL	0	NULL	suppliers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	For the healthcare industry , mobile applications provide a new frontier in offering better care and services to patients , and a more flexible and mobile way of communicating with suppliers and patients .
	manualset3
245343	9	427973	16	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	For the healthcare industry , mobile applications provide a new frontier in offering better care and services to patients , and a more flexible and mobile way of communicating with suppliers and patients .
	manualset3
245344	1	427974	16	NULL	NULL	NULL	NULL	hypothalamic response test	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For the hypothalamic response test , two basal samples ( 3.5 ml ) were collected at 15-min intervals via the saphenous vein , and then N-methyl-D-L-aspartic acid ( NMA ; 20 mg/kg ) was given iv and four more blood samples collected .
	manualset3
245345	2	427974	16	NULL	NULL	0	NULL	two basal samples	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the hypothalamic response test , two basal samples ( 3.5 ml ) were collected at 15-min intervals via the saphenous vein , and then N-methyl-D-L-aspartic acid ( NMA ; 20 mg/kg ) was given iv and four more blood samples collected .
	manualset3
245346	3	427974	16	NULL	NULL	0	NULL	3.5 ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the hypothalamic response test , two basal samples ( 3.5 ml ) were collected at 15-min intervals via the saphenous vein , and then N-methyl-D-L-aspartic acid ( NMA ; 20 mg/kg ) was given iv and four more blood samples collected .
	manualset3
245347	4	427974	16	NULL	NULL	0	NULL	15-min intervals	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	For the hypothalamic response test , two basal samples ( 3.5 ml ) were collected at 15-min intervals via the saphenous vein , and then N-methyl-D-L-aspartic acid ( NMA ; 20 mg/kg ) was given iv and four more blood samples collected .
	manualset3
245348	5	427974	16	NULL	NULL	0	NULL	saphenous vein	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	For the hypothalamic response test , two basal samples ( 3.5 ml ) were collected at 15-min intervals via the saphenous vein , and then N-methyl-D-L-aspartic acid ( NMA ; 20 mg/kg ) was given iv and four more blood samples collected .
	manualset3
245349	6	427974	16	NULL	NULL	NULL	NULL	N-methyl-D-L-aspartic acid ( NMA	SmallMolecule												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For the hypothalamic response test , two basal samples ( 3.5 ml ) were collected at 15-min intervals via the saphenous vein , and then N-methyl-D-L-aspartic acid ( NMA ; 20 mg/kg ) was given iv and four more blood samples collected .
	manualset3
245350	7	427974	16	NULL	NULL	0	NULL	20 mg/kg	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the hypothalamic response test , two basal samples ( 3.5 ml ) were collected at 15-min intervals via the saphenous vein , and then N-methyl-D-L-aspartic acid ( NMA ; 20 mg/kg ) was given iv and four more blood samples collected .
	manualset3
245351	8	427974	16	NULL	NULL	0	NULL	iv	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For the hypothalamic response test , two basal samples ( 3.5 ml ) were collected at 15-min intervals via the saphenous vein , and then N-methyl-D-L-aspartic acid ( NMA ; 20 mg/kg ) was given iv and four more blood samples collected .
	manualset3
245352	9	427974	16	NULL	NULL	0	NULL	four	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the hypothalamic response test , two basal samples ( 3.5 ml ) were collected at 15-min intervals via the saphenous vein , and then N-methyl-D-L-aspartic acid ( NMA ; 20 mg/kg ) was given iv and four more blood samples collected .
	manualset3
245353	10	427974	16	NULL	NULL	0	NULL	blood samples	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the hypothalamic response test , two basal samples ( 3.5 ml ) were collected at 15-min intervals via the saphenous vein , and then N-methyl-D-L-aspartic acid ( NMA ; 20 mg/kg ) was given iv and four more blood samples collected .
	manualset3
245354	1	427975	16	NULL	NULL	0	NULL	last decade	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	For the last decade , several Mendelian forms of PD have been identified .
	manualset3
245355	2	427975	16	NULL	NULL	0	NULL	Mendelian forms	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For the last decade , several Mendelian forms of PD have been identified .
	manualset3
245356	3	427975	16	NULL	NULL	0	NULL	PD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	For the last decade , several Mendelian forms of PD have been identified .
	manualset3
245357	1	427976	16	NULL	NULL	0	NULL	Renal cell carcinoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Renal cell carcinoma management and therapies in 2010 ) .
	manualset3
245358	2	427976	16	NULL	NULL	0	NULL	management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Renal cell carcinoma management and therapies in 2010 ) .
	manualset3
245359	3	427976	16	NULL	NULL	0	NULL	therapies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Renal cell carcinoma management and therapies in 2010 ) .
	manualset3
245360	4	427976	16	NULL	NULL	0	NULL	2010	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	( Renal cell carcinoma management and therapies in 2010 ) .
	manualset3
245361	1	427977	16	NULL	NULL	0	NULL	staff	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	For the leading staff of the institution the methodology is supplemented by the estimates of a number of intermediate indicators and their integral assessment which helps analyze the basic factors influencing the general level of physicians qualification .
	manualset3
245362	2	427977	16	NULL	NULL	0	NULL	institution	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	For the leading staff of the institution the methodology is supplemented by the estimates of a number of intermediate indicators and their integral assessment which helps analyze the basic factors influencing the general level of physicians qualification .
	manualset3
245363	3	427977	16	NULL	NULL	0	NULL	methodology	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the leading staff of the institution the methodology is supplemented by the estimates of a number of intermediate indicators and their integral assessment which helps analyze the basic factors influencing the general level of physicians qualification .
	manualset3
245364	4	427977	16	NULL	NULL	0	NULL	estimates	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the leading staff of the institution the methodology is supplemented by the estimates of a number of intermediate indicators and their integral assessment which helps analyze the basic factors influencing the general level of physicians qualification .
	manualset3
245365	5	427977	16	NULL	NULL	0	NULL	number	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the leading staff of the institution the methodology is supplemented by the estimates of a number of intermediate indicators and their integral assessment which helps analyze the basic factors influencing the general level of physicians qualification .
	manualset3
245366	6	427977	16	NULL	NULL	0	NULL	intermediate indicators	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	For the leading staff of the institution the methodology is supplemented by the estimates of a number of intermediate indicators and their integral assessment which helps analyze the basic factors influencing the general level of physicians qualification .
	manualset3
245367	7	427977	16	NULL	NULL	0	NULL	integral assessment	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the leading staff of the institution the methodology is supplemented by the estimates of a number of intermediate indicators and their integral assessment which helps analyze the basic factors influencing the general level of physicians qualification .
	manualset3
245368	8	427977	16	NULL	NULL	0	NULL	factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the leading staff of the institution the methodology is supplemented by the estimates of a number of intermediate indicators and their integral assessment which helps analyze the basic factors influencing the general level of physicians qualification .
	manualset3
245369	9	427977	16	NULL	NULL	0	NULL	general level	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the leading staff of the institution the methodology is supplemented by the estimates of a number of intermediate indicators and their integral assessment which helps analyze the basic factors influencing the general level of physicians qualification .
	manualset3
245370	10	427977	16	NULL	NULL	0	NULL	physicians	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	For the leading staff of the institution the methodology is supplemented by the estimates of a number of intermediate indicators and their integral assessment which helps analyze the basic factors influencing the general level of physicians qualification .
	manualset3
245371	11	427977	16	NULL	NULL	NULL	NULL	qualification	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For the leading staff of the institution the methodology is supplemented by the estimates of a number of intermediate indicators and their integral assessment which helps analyze the basic factors influencing the general level of physicians qualification .
	manualset3
245372	1	427978	16	NULL	NULL	NULL	NULL	mixture	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For the mixture , the median maximal level of CsA in whole saliva was 2867 ng/ml compared to 5.4 ng/ml for the capsule .
	manualset3
245373	2	427978	16	NULL	NULL	NULL	NULL	median maximal level of CsA	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For the mixture , the median maximal level of CsA in whole saliva was 2867 ng/ml compared to 5.4 ng/ml for the capsule .
	manualset3
245374	3	427978	16	NULL	NULL	0	NULL	saliva	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	For the mixture , the median maximal level of CsA in whole saliva was 2867 ng/ml compared to 5.4 ng/ml for the capsule .
	manualset3
245375	4	427978	16	NULL	NULL	0	NULL	2867 ng/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the mixture , the median maximal level of CsA in whole saliva was 2867 ng/ml compared to 5.4 ng/ml for the capsule .
	manualset3
245376	5	427978	16	NULL	NULL	0	NULL	5.4 ng/ml	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the mixture , the median maximal level of CsA in whole saliva was 2867 ng/ml compared to 5.4 ng/ml for the capsule .
	manualset3
245377	6	427978	16	NULL	NULL	NULL	NULL	capsule	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For the mixture , the median maximal level of CsA in whole saliva was 2867 ng/ml compared to 5.4 ng/ml for the capsule .
	manualset3
245378	1	427979	16	NULL	NULL	0	NULL	objective lenses	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	For the objective lenses investigated , we observed pulse broadening on the order of around 4 % -7 % for air immersion lenses and 9 % -12 % for oil immersion lenses .
	manualset3
245383	2	427979	16	NULL	NULL	0	NULL	pulse broadening	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the objective lenses investigated , we observed pulse broadening on the order of around 4 % -7 % for air immersion lenses and 9 % -12 % for oil immersion lenses .
	manualset3
245388	3	427979	16	NULL	NULL	0	NULL	order	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the objective lenses investigated , we observed pulse broadening on the order of around 4 % -7 % for air immersion lenses and 9 % -12 % for oil immersion lenses .
	manualset3
245390	4	427979	16	NULL	NULL	0	NULL	4 % -7 %	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the objective lenses investigated , we observed pulse broadening on the order of around 4 % -7 % for air immersion lenses and 9 % -12 % for oil immersion lenses .
	manualset3
245393	5	427979	16	NULL	NULL	0	NULL	air immersion lenses	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	For the objective lenses investigated , we observed pulse broadening on the order of around 4 % -7 % for air immersion lenses and 9 % -12 % for oil immersion lenses .
	manualset3
245394	6	427979	16	NULL	NULL	0	NULL	9 % -12 %	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the objective lenses investigated , we observed pulse broadening on the order of around 4 % -7 % for air immersion lenses and 9 % -12 % for oil immersion lenses .
	manualset3
245395	7	427979	16	NULL	NULL	0	NULL	oil immersion lenses	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	For the objective lenses investigated , we observed pulse broadening on the order of around 4 % -7 % for air immersion lenses and 9 % -12 % for oil immersion lenses .
	manualset3
245444	1	427980	16	NULL	NULL	0	NULL	decades	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	For the past several decades , we have been able to directly probe the motion of atoms that is associated with chemical transformations and which occurs on the femtosecond ( 10 ( -15 ) - s ) timescale .
	manualset3
245446	2	427980	16	NULL	NULL	0	NULL	motion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For the past several decades , we have been able to directly probe the motion of atoms that is associated with chemical transformations and which occurs on the femtosecond ( 10 ( -15 ) - s ) timescale .
	manualset3
245447	3	427980	16	NULL	NULL	0	NULL	atoms	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	For the past several decades , we have been able to directly probe the motion of atoms that is associated with chemical transformations and which occurs on the femtosecond ( 10 ( -15 ) - s ) timescale .
	manualset3
245449	4	427980	16	NULL	NULL	0	NULL	chemical transformations	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	For the past several decades , we have been able to directly probe the motion of atoms that is associated with chemical transformations and which occurs on the femtosecond ( 10 ( -15 ) - s ) timescale .
	manualset3
245451	5	427980	16	NULL	NULL	0	NULL	femtosecond ( 10 ( -15 ) - s ) timescale	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the past several decades , we have been able to directly probe the motion of atoms that is associated with chemical transformations and which occurs on the femtosecond ( 10 ( -15 ) - s ) timescale .
	manualset3
245258	1	427981	16	NULL	NULL	NULL	NULL	prediction	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For the prediction of sensory tenderness , the WBSF standard procedure ( protocol A ) showed the lowest variance ( R ( 2 ) = 15 % ) and the highest standard error of the estimate ( SEE = 0.97 N ) compared to the other WBSF protocols .
	manualset3
245485	2	427981	16	NULL	NULL	0	NULL	sensory tenderness	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the prediction of sensory tenderness , the WBSF standard procedure ( protocol A ) showed the lowest variance ( R ( 2 ) = 15 % ) and the highest standard error of the estimate ( SEE = 0.97 N ) compared to the other WBSF protocols .
	manualset3
245486	3	427981	16	NULL	NULL	0	NULL	WBSF standard procedure ( protocol A )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the prediction of sensory tenderness , the WBSF standard procedure ( protocol A ) showed the lowest variance ( R ( 2 ) = 15 % ) and the highest standard error of the estimate ( SEE = 0.97 N ) compared to the other WBSF protocols .
	manualset3
245488	4	427981	16	NULL	NULL	0	NULL	variance	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the prediction of sensory tenderness , the WBSF standard procedure ( protocol A ) showed the lowest variance ( R ( 2 ) = 15 % ) and the highest standard error of the estimate ( SEE = 0.97 N ) compared to the other WBSF protocols .
	manualset3
245490	5	427981	16	NULL	NULL	0	NULL	R ( 2 ) = 15 %	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the prediction of sensory tenderness , the WBSF standard procedure ( protocol A ) showed the lowest variance ( R ( 2 ) = 15 % ) and the highest standard error of the estimate ( SEE = 0.97 N ) compared to the other WBSF protocols .
	manualset3
245492	6	427981	16	NULL	NULL	0	NULL	standard error of the estimate ( SEE	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the prediction of sensory tenderness , the WBSF standard procedure ( protocol A ) showed the lowest variance ( R ( 2 ) = 15 % ) and the highest standard error of the estimate ( SEE = 0.97 N ) compared to the other WBSF protocols .
	manualset3
245493	7	427981	16	NULL	NULL	0	NULL	0.97 N	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the prediction of sensory tenderness , the WBSF standard procedure ( protocol A ) showed the lowest variance ( R ( 2 ) = 15 % ) and the highest standard error of the estimate ( SEE = 0.97 N ) compared to the other WBSF protocols .
	manualset3
245496	8	427981	16	NULL	NULL	0	NULL	WBSF protocols	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the prediction of sensory tenderness , the WBSF standard procedure ( protocol A ) showed the lowest variance ( R ( 2 ) = 15 % ) and the highest standard error of the estimate ( SEE = 0.97 N ) compared to the other WBSF protocols .
	manualset3
245505	1	427982	16	NULL	NULL	0	NULL	chloroplast phosphorylase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For the purified chloroplast phosphorylase , sodium dodecyl-sulfate polyacrylamide gel electrophoresis and pyridoxal phosphate determination resulted in a molecular weight estimation of about 110 , 000 per monomer .
	manualset3
245509	2	427982	16	NULL	NULL	0	NULL	sodium dodecyl-sulfate polyacrylamide gel electrophoresis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the purified chloroplast phosphorylase , sodium dodecyl-sulfate polyacrylamide gel electrophoresis and pyridoxal phosphate determination resulted in a molecular weight estimation of about 110 , 000 per monomer .
	manualset3
245510	3	427982	16	NULL	NULL	0	NULL	pyridoxal phosphate determination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the purified chloroplast phosphorylase , sodium dodecyl-sulfate polyacrylamide gel electrophoresis and pyridoxal phosphate determination resulted in a molecular weight estimation of about 110 , 000 per monomer .
	manualset3
245512	4	427982	16	NULL	NULL	0	NULL	molecular weight estimation	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the purified chloroplast phosphorylase , sodium dodecyl-sulfate polyacrylamide gel electrophoresis and pyridoxal phosphate determination resulted in a molecular weight estimation of about 110 , 000 per monomer .
	manualset3
245515	1	427983	16	NULL	NULL	0	NULL	quinonoid complex	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For the quinonoid complex with erythro-3-hydroxyaspartate , the tilt angles were found to be 63 degrees in cAAT and 53 degrees in mAAT .
	manualset3
245516	2	427983	16	NULL	NULL	0	NULL	erythro-3-hydroxyaspartate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For the quinonoid complex with erythro-3-hydroxyaspartate , the tilt angles were found to be 63 degrees in cAAT and 53 degrees in mAAT .
	manualset3
245517	3	427983	16	NULL	NULL	0	NULL	tilt angles	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the quinonoid complex with erythro-3-hydroxyaspartate , the tilt angles were found to be 63 degrees in cAAT and 53 degrees in mAAT .
	manualset3
245518	4	427983	16	NULL	NULL	0	NULL	63 degrees	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the quinonoid complex with erythro-3-hydroxyaspartate , the tilt angles were found to be 63 degrees in cAAT and 53 degrees in mAAT .
	manualset3
245532	5	427983	16	NULL	NULL	0	NULL	cAAT	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For the quinonoid complex with erythro-3-hydroxyaspartate , the tilt angles were found to be 63 degrees in cAAT and 53 degrees in mAAT .
	manualset3
245533	6	427983	16	NULL	NULL	0	NULL	53 degrees	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the quinonoid complex with erythro-3-hydroxyaspartate , the tilt angles were found to be 63 degrees in cAAT and 53 degrees in mAAT .
	manualset3
245534	7	427983	16	NULL	NULL	0	NULL	mAAT	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For the quinonoid complex with erythro-3-hydroxyaspartate , the tilt angles were found to be 63 degrees in cAAT and 53 degrees in mAAT .
	manualset3
245535	1	427984	16	NULL	NULL	0	NULL	Renal changes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Renal changes in scleroderma ) .
	manualset3
245536	2	427984	16	NULL	NULL	0	NULL	scleroderma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Renal changes in scleroderma ) .
	manualset3
245514	5	427985	16	NULL	NULL	NULL	NULL	increases	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For the same reason , EPS accumulation can fall as its rate of production increases .
	manualset3
245537	1	427985	16	NULL	NULL	NULL	NULL	EPS accumulation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For the same reason , EPS accumulation can fall as its rate of production increases .
	manualset3
245538	2	427985	16	NULL	NULL	0	NULL	rate of production	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the same reason , EPS accumulation can fall as its rate of production increases .
	manualset3
250109	6	427985	16	NULL	NULL	0	NULL	reason	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the same reason , EPS accumulation can fall as its rate of production increases .
	manualset3
245539	1	427986	16	NULL	NULL	NULL	NULL	symptom	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For the symptom common to both assessment methods ( dryness ) , there is a good correlation between the two methods ( Spearman 's Rho : P = 0.032 ) .
	manualset3
245540	2	427986	16	NULL	NULL	0	NULL	assessment methods	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the symptom common to both assessment methods ( dryness ) , there is a good correlation between the two methods ( Spearman 's Rho : P = 0.032 ) .
	manualset3
245541	3	427986	16	NULL	NULL	0	NULL	dryness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For the symptom common to both assessment methods ( dryness ) , there is a good correlation between the two methods ( Spearman 's Rho : P = 0.032 ) .
	manualset3
245542	4	427986	16	NULL	NULL	0	NULL	correlation	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	For the symptom common to both assessment methods ( dryness ) , there is a good correlation between the two methods ( Spearman 's Rho : P = 0.032 ) .
	manualset3
245543	5	427986	16	NULL	NULL	0	NULL	two methods	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For the symptom common to both assessment methods ( dryness ) , there is a good correlation between the two methods ( Spearman 's Rho : P = 0.032 ) .
	manualset3
245544	6	427986	16	NULL	NULL	0	NULL	Spearman 's Rho : P = 0.032	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For the symptom common to both assessment methods ( dryness ) , there is a good correlation between the two methods ( Spearman 's Rho : P = 0.032 ) .
	manualset3
245550	1	427987	16	NULL	NULL	0	NULL	termination	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For the termination of paroxysmal supraventricular tachycardia , intravenous administration of verapamil or aprindine was more effective than that of disopyramide or procainamide .
	manualset3
245553	2	427987	16	NULL	NULL	0	NULL	paroxysmal supraventricular tachycardia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For the termination of paroxysmal supraventricular tachycardia , intravenous administration of verapamil or aprindine was more effective than that of disopyramide or procainamide .
	manualset3
245554	3	427987	16	NULL	NULL	0	NULL	intravenous administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For the termination of paroxysmal supraventricular tachycardia , intravenous administration of verapamil or aprindine was more effective than that of disopyramide or procainamide .
	manualset3
245555	4	427987	16	NULL	NULL	0	NULL	verapamil	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	For the termination of paroxysmal supraventricular tachycardia , intravenous administration of verapamil or aprindine was more effective than that of disopyramide or procainamide .
	manualset3
245556	5	427987	16	NULL	NULL	0	NULL	aprindine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	For the termination of paroxysmal supraventricular tachycardia , intravenous administration of verapamil or aprindine was more effective than that of disopyramide or procainamide .
	manualset3
245560	6	427987	16	NULL	NULL	0	NULL	disopyramide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	For the termination of paroxysmal supraventricular tachycardia , intravenous administration of verapamil or aprindine was more effective than that of disopyramide or procainamide .
	manualset3
245562	7	427987	16	NULL	NULL	0	NULL	procainamide	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	For the termination of paroxysmal supraventricular tachycardia , intravenous administration of verapamil or aprindine was more effective than that of disopyramide or procainamide .
	manualset3
245567	1	427988	16	NULL	NULL	0	NULL	23	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For these 23 isolates , MICs were 8g/mL for ceftriaxone , 4-8g / mL for penicillin and 0.5-2g / mL for ceftobiprole .
	manualset3
245569	2	427988	16	NULL	NULL	0	NULL	isolates	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For these 23 isolates , MICs were 8g/mL for ceftriaxone , 4-8g / mL for penicillin and 0.5-2g / mL for ceftobiprole .
	manualset3
245570	3	427988	16	NULL	NULL	0	NULL	MICs	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For these 23 isolates , MICs were 8g/mL for ceftriaxone , 4-8g / mL for penicillin and 0.5-2g / mL for ceftobiprole .
	manualset3
245571	4	427988	16	NULL	NULL	0	NULL	8g/mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For these 23 isolates , MICs were 8g/mL for ceftriaxone , 4-8g / mL for penicillin and 0.5-2g / mL for ceftobiprole .
	manualset3
245572	5	427988	16	NULL	NULL	0	NULL	ceftriaxone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	For these 23 isolates , MICs were 8g/mL for ceftriaxone , 4-8g / mL for penicillin and 0.5-2g / mL for ceftobiprole .
	manualset3
245573	6	427988	16	NULL	NULL	0	NULL	4-8g / mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For these 23 isolates , MICs were 8g/mL for ceftriaxone , 4-8g / mL for penicillin and 0.5-2g / mL for ceftobiprole .
	manualset3
245574	7	427988	16	NULL	NULL	0	NULL	penicillin	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	For these 23 isolates , MICs were 8g/mL for ceftriaxone , 4-8g / mL for penicillin and 0.5-2g / mL for ceftobiprole .
	manualset3
245575	8	427988	16	NULL	NULL	0	NULL	0.5-2g / mL	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For these 23 isolates , MICs were 8g/mL for ceftriaxone , 4-8g / mL for penicillin and 0.5-2g / mL for ceftobiprole .
	manualset3
245576	9	427988	16	NULL	NULL	0	NULL	ceftobiprole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	For these 23 isolates , MICs were 8g/mL for ceftriaxone , 4-8g / mL for penicillin and 0.5-2g / mL for ceftobiprole .
	manualset3
245577	1	427989	16	NULL	NULL	0	NULL	concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For this aim , different concentrations ( 1 , 2 , 5 , 10 and 20 mM ) of benomyl solutions were used .
	manualset3
245578	2	427989	16	NULL	NULL	0	NULL	1 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For this aim , different concentrations ( 1 , 2 , 5 , 10 and 20 mM ) of benomyl solutions were used .
	manualset3
245579	3	427989	16	NULL	NULL	0	NULL	2 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For this aim , different concentrations ( 1 , 2 , 5 , 10 and 20 mM ) of benomyl solutions were used .
	manualset3
245580	4	427989	16	NULL	NULL	0	NULL	5 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For this aim , different concentrations ( 1 , 2 , 5 , 10 and 20 mM ) of benomyl solutions were used .
	manualset3
245581	5	427989	16	NULL	NULL	0	NULL	10 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For this aim , different concentrations ( 1 , 2 , 5 , 10 and 20 mM ) of benomyl solutions were used .
	manualset3
245582	6	427989	16	NULL	NULL	0	NULL	20 mM	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For this aim , different concentrations ( 1 , 2 , 5 , 10 and 20 mM ) of benomyl solutions were used .
	manualset3
245583	7	427989	16	NULL	NULL	0	NULL	benomyl solutions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For this aim , different concentrations ( 1 , 2 , 5 , 10 and 20 mM ) of benomyl solutions were used .
	manualset3
245584	1	427990	16	NULL	NULL	0	NULL	intradermal test	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For this purpose , intradermal test with protein purified derivative , dinitrochlorobenzene , test of migration inhibitory factor with protein purified derivative and candidin antigens and cutaneous window were performed .
	manualset3
245585	2	427990	16	NULL	NULL	NULL	NULL	protein purified derivative	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For this purpose , intradermal test with protein purified derivative , dinitrochlorobenzene , test of migration inhibitory factor with protein purified derivative and candidin antigens and cutaneous window were performed .
	manualset3
245586	3	427990	16	NULL	NULL	0	NULL	dinitrochlorobenzene	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For this purpose , intradermal test with protein purified derivative , dinitrochlorobenzene , test of migration inhibitory factor with protein purified derivative and candidin antigens and cutaneous window were performed .
	manualset3
245587	4	427990	16	NULL	NULL	0	NULL	test of migration inhibitory factor	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For this purpose , intradermal test with protein purified derivative , dinitrochlorobenzene , test of migration inhibitory factor with protein purified derivative and candidin antigens and cutaneous window were performed .
	manualset3
245588	5	427990	16	NULL	NULL	NULL	NULL	protein purified derivative	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For this purpose , intradermal test with protein purified derivative , dinitrochlorobenzene , test of migration inhibitory factor with protein purified derivative and candidin antigens and cutaneous window were performed .
	manualset3
245589	6	427990	16	NULL	NULL	0	NULL	candidin antigens	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For this purpose , intradermal test with protein purified derivative , dinitrochlorobenzene , test of migration inhibitory factor with protein purified derivative and candidin antigens and cutaneous window were performed .
	manualset3
245590	7	427990	16	NULL	NULL	0	NULL	cutaneous window	MedicalProcedureOrDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	For this purpose , intradermal test with protein purified derivative , dinitrochlorobenzene , test of migration inhibitory factor with protein purified derivative and candidin antigens and cutaneous window were performed .
	manualset3
251794	8	427990	16	NULL	NULL	0	NULL	purpose	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For this purpose , intradermal test with protein purified derivative , dinitrochlorobenzene , test of migration inhibitory factor with protein purified derivative and candidin antigens and cutaneous window were performed .
	manualset3
245591	1	427991	16	NULL	NULL	0	NULL	skin pieces	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	For this purpose skin pieces are cultured for several days and migratory DC emigrate from epidermis and dermis .
	manualset3
245592	2	427991	16	NULL	NULL	0	NULL	days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	For this purpose skin pieces are cultured for several days and migratory DC emigrate from epidermis and dermis .
	manualset3
245593	3	427991	16	NULL	NULL	0	NULL	migratory DC	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	For this purpose skin pieces are cultured for several days and migratory DC emigrate from epidermis and dermis .
	manualset3
245594	4	427991	16	NULL	NULL	0	NULL	epidermis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	For this purpose skin pieces are cultured for several days and migratory DC emigrate from epidermis and dermis .
	manualset3
245595	5	427991	16	NULL	NULL	0	NULL	dermis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	For this purpose skin pieces are cultured for several days and migratory DC emigrate from epidermis and dermis .
	manualset3
245596	1	427992	16	NULL	NULL	0	NULL	levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason , it is critical to accurately characterize both the levels and the sites of Asn deamidation in therapeutic antibodies .
	manualset3
245597	2	427992	16	NULL	NULL	NULL	NULL	sites	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For this reason , it is critical to accurately characterize both the levels and the sites of Asn deamidation in therapeutic antibodies .
	manualset3
245598	3	427992	16	NULL	NULL	NULL	NULL	Asn deamidation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For this reason , it is critical to accurately characterize both the levels and the sites of Asn deamidation in therapeutic antibodies .
	manualset3
245599	4	427992	16	NULL	NULL	NULL	NULL	reason	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For this reason , it is critical to accurately characterize both the levels and the sites of Asn deamidation in therapeutic antibodies .
	manualset3
245600	5	427992	16	NULL	NULL	0	NULL	therapeutic antibodies	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason , it is critical to accurately characterize both the levels and the sites of Asn deamidation in therapeutic antibodies .
	manualset3
245601	1	427993	16	NULL	NULL	NULL	NULL	mechanisms	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For this reason , it is important to determine the mechanisms that act to regulate TDP-43 levels within the cell .
	manualset3
245606	2	427993	16	NULL	NULL	0	NULL	TDP-43	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason , it is important to determine the mechanisms that act to regulate TDP-43 levels within the cell .
	manualset3
245609	3	427993	16	NULL	NULL	0	NULL	levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason , it is important to determine the mechanisms that act to regulate TDP-43 levels within the cell .
	manualset3
245610	4	427993	16	NULL	NULL	0	NULL	cell	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason , it is important to determine the mechanisms that act to regulate TDP-43 levels within the cell .
	manualset3
245612	1	427994	16	NULL	NULL	0	NULL	structural elucidation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason , the structural elucidation of lipopolysaccharides from toxic Gram-negative bacteria is an important and complicated task , mainly owing to its natural heterogeneity .
	manualset3
245614	2	427994	16	NULL	NULL	0	NULL	lipopolysaccharides	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason , the structural elucidation of lipopolysaccharides from toxic Gram-negative bacteria is an important and complicated task , mainly owing to its natural heterogeneity .
	manualset3
245616	3	427994	16	NULL	NULL	0	NULL	toxic Gram-negative bacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason , the structural elucidation of lipopolysaccharides from toxic Gram-negative bacteria is an important and complicated task , mainly owing to its natural heterogeneity .
	manualset3
245621	4	427994	16	NULL	NULL	NULL	NULL	task	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For this reason , the structural elucidation of lipopolysaccharides from toxic Gram-negative bacteria is an important and complicated task , mainly owing to its natural heterogeneity .
	manualset3
245625	5	427994	16	NULL	NULL	NULL	NULL	heterogeneity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For this reason , the structural elucidation of lipopolysaccharides from toxic Gram-negative bacteria is an important and complicated task , mainly owing to its natural heterogeneity .
	manualset3
251795	6	427994	16	NULL	NULL	0	NULL	reason	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason , the structural elucidation of lipopolysaccharides from toxic Gram-negative bacteria is an important and complicated task , mainly owing to its natural heterogeneity .
	manualset3
245627	1	427995	16	NULL	NULL	0	NULL	 immunohistochemical study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason , we performed an immunohistochemical study using human cardiac muscle fibers , in order to define the real distribution and the spatial relationship between the proteins in these two complexes .
	manualset3
245630	2	427995	16	NULL	NULL	0	NULL	human cardiac muscle fibers	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason , we performed an immunohistochemical study using human cardiac muscle fibers , in order to define the real distribution and the spatial relationship between the proteins in these two complexes .
	manualset3
245632	3	427995	16	NULL	NULL	0	NULL	distribution	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason , we performed an immunohistochemical study using human cardiac muscle fibers , in order to define the real distribution and the spatial relationship between the proteins in these two complexes .
	manualset3
245634	4	427995	16	NULL	NULL	0	NULL	spatial relationship	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason , we performed an immunohistochemical study using human cardiac muscle fibers , in order to define the real distribution and the spatial relationship between the proteins in these two complexes .
	manualset3
245636	5	427995	16	NULL	NULL	0	NULL	proteins	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason , we performed an immunohistochemical study using human cardiac muscle fibers , in order to define the real distribution and the spatial relationship between the proteins in these two complexes .
	manualset3
245638	6	427995	16	NULL	NULL	0	NULL	two complexes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason , we performed an immunohistochemical study using human cardiac muscle fibers , in order to define the real distribution and the spatial relationship between the proteins in these two complexes .
	manualset3
245641	1	427996	16	NULL	NULL	0	NULL	laparoscopic 180-degree anterior fundoplication	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason we have investigated the use of a laparoscopic 180-degree anterior fundoplication as a technique that has the potential to control reflux , but with less associated postoperative dysphagia and fewer gas-related side effects .
	manualset3
245644	2	427996	16	NULL	NULL	0	NULL	technique	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason we have investigated the use of a laparoscopic 180-degree anterior fundoplication as a technique that has the potential to control reflux , but with less associated postoperative dysphagia and fewer gas-related side effects .
	manualset3
245647	3	427996	16	NULL	NULL	NULL	NULL	potential	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For this reason we have investigated the use of a laparoscopic 180-degree anterior fundoplication as a technique that has the potential to control reflux , but with less associated postoperative dysphagia and fewer gas-related side effects .
	manualset3
245649	4	427996	16	NULL	NULL	0	NULL	reflux	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason we have investigated the use of a laparoscopic 180-degree anterior fundoplication as a technique that has the potential to control reflux , but with less associated postoperative dysphagia and fewer gas-related side effects .
	manualset3
245657	5	427996	16	NULL	NULL	0	NULL	postoperative dysphagia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason we have investigated the use of a laparoscopic 180-degree anterior fundoplication as a technique that has the potential to control reflux , but with less associated postoperative dysphagia and fewer gas-related side effects .
	manualset3
245659	6	427996	16	NULL	NULL	0	NULL	gas-related side effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason we have investigated the use of a laparoscopic 180-degree anterior fundoplication as a technique that has the potential to control reflux , but with less associated postoperative dysphagia and fewer gas-related side effects .
	manualset3
247062	7	427996	16	NULL	NULL	0	NULL	reason	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason we have investigated the use of a laparoscopic 180-degree anterior fundoplication as a technique that has the potential to control reflux , but with less associated postoperative dysphagia and fewer gas-related side effects .
	manualset3
247063	8	427996	16	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason we have investigated the use of a laparoscopic 180-degree anterior fundoplication as a technique that has the potential to control reflux , but with less associated postoperative dysphagia and fewer gas-related side effects .
	manualset3
245664	1	427997	16	NULL	NULL	0	NULL	relationship	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason we investigated the relationship between retinal structural lesions and quantitative measures of glomerular structure in patients with insulin-dependent diabetes mellitus ( IDDM ) .
	manualset3
245666	2	427997	16	NULL	NULL	0	NULL	retinal structural lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason we investigated the relationship between retinal structural lesions and quantitative measures of glomerular structure in patients with insulin-dependent diabetes mellitus ( IDDM ) .
	manualset3
245668	3	427997	16	NULL	NULL	0	NULL	quantitative measures	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason we investigated the relationship between retinal structural lesions and quantitative measures of glomerular structure in patients with insulin-dependent diabetes mellitus ( IDDM ) .
	manualset3
245670	4	427997	16	NULL	NULL	0	NULL	glomerular structure	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason we investigated the relationship between retinal structural lesions and quantitative measures of glomerular structure in patients with insulin-dependent diabetes mellitus ( IDDM ) .
	manualset3
245671	5	427997	16	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason we investigated the relationship between retinal structural lesions and quantitative measures of glomerular structure in patients with insulin-dependent diabetes mellitus ( IDDM ) .
	manualset3
245672	6	427997	16	NULL	NULL	0	NULL	insulin-dependent diabetes mellitus ( IDDM )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	For this reason we investigated the relationship between retinal structural lesions and quantitative measures of glomerular structure in patients with insulin-dependent diabetes mellitus ( IDDM ) .
	manualset3
245676	1	427998	16	NULL	NULL	0	NULL	Renovascular hypertension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Renovascular hypertension : angioplasty need not be essential ) .
	manualset3
245677	2	427998	16	NULL	NULL	0	NULL	angioplasty	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Renovascular hypertension : angioplasty need not be essential ) .
	manualset3
245680	1	427999	16	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	For those patients unresponsive to standard treatment regimens , liver transplantation may be the only suitable treatment option .
	manualset3
245683	2	427999	16	NULL	NULL	0	NULL	standard treatment regimens	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For those patients unresponsive to standard treatment regimens , liver transplantation may be the only suitable treatment option .
	manualset3
245686	3	427999	16	NULL	NULL	0	NULL	liver transplantation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For those patients unresponsive to standard treatment regimens , liver transplantation may be the only suitable treatment option .
	manualset3
245688	4	427999	16	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	For those patients unresponsive to standard treatment regimens , liver transplantation may be the only suitable treatment option .
	manualset3
245690	5	427999	16	NULL	NULL	0	NULL	option	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	For those patients unresponsive to standard treatment regimens , liver transplantation may be the only suitable treatment option .
	manualset3
245691	1	428000	16	NULL	NULL	0	NULL	data	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For updated information , including data and facts on specific diseases , visit ( http : //www.health.nsw.gov.au ) and click on Infectious Diseases .
	manualset3
245692	2	428000	16	NULL	NULL	0	NULL	facts	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For updated information , including data and facts on specific diseases , visit ( http : //www.health.nsw.gov.au ) and click on Infectious Diseases .
	manualset3
245693	3	428000	16	NULL	NULL	0	NULL	diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	For updated information , including data and facts on specific diseases , visit ( http : //www.health.nsw.gov.au ) and click on Infectious Diseases .
	manualset3
245694	4	428000	16	NULL	NULL	0	NULL	 http : //www.health.nsw.gov.au	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	For updated information , including data and facts on specific diseases , visit ( http : //www.health.nsw.gov.au ) and click on Infectious Diseases .
	manualset3
245695	5	428000	16	NULL	NULL	0	NULL	Infectious Diseases	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	For updated information , including data and facts on specific diseases , visit ( http : //www.health.nsw.gov.au ) and click on Infectious Diseases .
	manualset3
250144	6	428000	16	NULL	NULL	NULL	NULL	updated information	PublishedSourceOfInformation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For updated information , including data and facts on specific diseases , visit ( http : //www.health.nsw.gov.au ) and click on Infectious Diseases .
	manualset3
245696	1	428001	16	NULL	NULL	NULL	NULL	question	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For us , the question of when to operate for osteolysis remains unanswered .
	manualset3
245697	2	428001	16	NULL	NULL	0	NULL	osteolysis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	For us , the question of when to operate for osteolysis remains unanswered .
	manualset3
245698	1	428002	16	NULL	NULL	0	NULL	validation purposes	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For validation purposes , the compounds were quantified in water and 95 % ethanol and the results showed high sensitivity , good precision and accuracy .
	manualset3
245699	2	428002	16	NULL	NULL	0	NULL	compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For validation purposes , the compounds were quantified in water and 95 % ethanol and the results showed high sensitivity , good precision and accuracy .
	manualset3
245700	3	428002	16	NULL	NULL	0	NULL	water	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	For validation purposes , the compounds were quantified in water and 95 % ethanol and the results showed high sensitivity , good precision and accuracy .
	manualset3
245701	4	428002	16	NULL	NULL	NULL	NULL	95 % ethanol	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For validation purposes , the compounds were quantified in water and 95 % ethanol and the results showed high sensitivity , good precision and accuracy .
	manualset3
245703	6	428002	16	NULL	NULL	NULL	NULL	results	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For validation purposes , the compounds were quantified in water and 95 % ethanol and the results showed high sensitivity , good precision and accuracy .
	manualset3
245704	7	428002	16	NULL	NULL	0	NULL	sensitivity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For validation purposes , the compounds were quantified in water and 95 % ethanol and the results showed high sensitivity , good precision and accuracy .
	manualset3
245705	8	428002	16	NULL	NULL	0	NULL	precision	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For validation purposes , the compounds were quantified in water and 95 % ethanol and the results showed high sensitivity , good precision and accuracy .
	manualset3
245706	9	428002	16	NULL	NULL	0	NULL	accuracy	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	For validation purposes , the compounds were quantified in water and 95 % ethanol and the results showed high sensitivity , good precision and accuracy .
	manualset3
245708	2	428003	16	NULL	NULL	NULL	NULL	groups of strains	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For various groups of strains sharing the same serotype ( e.g. 4b , 1/2a , 1/2b ) , RAPD analysis could generate further subdivision .
	manualset3
245709	3	428003	16	NULL	NULL	NULL	NULL	serotype 4b	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For various groups of strains sharing the same serotype ( e.g. 4b , 1/2a , 1/2b ) , RAPD analysis could generate further subdivision .
	manualset3
245710	4	428003	16	NULL	NULL	0	NULL	serotype 1/2a	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For various groups of strains sharing the same serotype ( e.g. 4b , 1/2a , 1/2b ) , RAPD analysis could generate further subdivision .
	manualset3
245711	5	428003	16	NULL	NULL	0	NULL	serotype 1/2b	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	For various groups of strains sharing the same serotype ( e.g. 4b , 1/2a , 1/2b ) , RAPD analysis could generate further subdivision .
	manualset3
245712	6	428003	16	NULL	NULL	0	NULL	RAPD analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	For various groups of strains sharing the same serotype ( e.g. 4b , 1/2a , 1/2b ) , RAPD analysis could generate further subdivision .
	manualset3
245713	7	428003	16	NULL	NULL	NULL	NULL	subdivision	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	For various groups of strains sharing the same serotype ( e.g. 4b , 1/2a , 1/2b ) , RAPD analysis could generate further subdivision .
	manualset3
245714	1	428004	16	NULL	NULL	0	NULL	Reoperations	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Reoperations of the thyroid gland ) .
	manualset3
245715	2	428004	16	NULL	NULL	0	NULL	thyroid gland	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Reoperations of the thyroid gland ) .
	manualset3
245716	1	428005	16	NULL	NULL	NULL	NULL	Foramen nutritium radii ( FNR )	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Foramen nutritium radii ( FNR ) and foramen nutritium ulnae ( FNU ) were located mainly along facies anterior and its edges margo anterior and margo interosseus and only in a few cases they were observed along facies posterior .
	manualset3
245717	2	428005	16	NULL	NULL	NULL	NULL	oramen nutritium ulnae ( FNU )	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Foramen nutritium radii ( FNR ) and foramen nutritium ulnae ( FNU ) were located mainly along facies anterior and its edges margo anterior and margo interosseus and only in a few cases they were observed along facies posterior .
	manualset3
245718	3	428005	16	NULL	NULL	NULL	NULL	facies anterior	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Foramen nutritium radii ( FNR ) and foramen nutritium ulnae ( FNU ) were located mainly along facies anterior and its edges margo anterior and margo interosseus and only in a few cases they were observed along facies posterior .
	manualset3
245719	4	428005	16	NULL	NULL	NULL	NULL	margo anterior	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Foramen nutritium radii ( FNR ) and foramen nutritium ulnae ( FNU ) were located mainly along facies anterior and its edges margo anterior and margo interosseus and only in a few cases they were observed along facies posterior .
	manualset3
245720	5	428005	16	NULL	NULL	NULL	NULL	margo interosseus	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Foramen nutritium radii ( FNR ) and foramen nutritium ulnae ( FNU ) were located mainly along facies anterior and its edges margo anterior and margo interosseus and only in a few cases they were observed along facies posterior .
	manualset3
245721	6	428005	16	NULL	NULL	NULL	NULL	few cases	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Foramen nutritium radii ( FNR ) and foramen nutritium ulnae ( FNU ) were located mainly along facies anterior and its edges margo anterior and margo interosseus and only in a few cases they were observed along facies posterior .
	manualset3
245722	7	428005	16	NULL	NULL	NULL	NULL	facies posterior	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Foramen nutritium radii ( FNR ) and foramen nutritium ulnae ( FNU ) were located mainly along facies anterior and its edges margo anterior and margo interosseus and only in a few cases they were observed along facies posterior .
	manualset3
245723	1	428006	16	NULL	NULL	0	NULL	Force-stabilization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Force-stabilization by all eight fingers improved quantitatively with practice .
	manualset3
245724	2	428006	16	NULL	NULL	0	NULL	eight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Force-stabilization by all eight fingers improved quantitatively with practice .
	manualset3
245725	3	428006	16	NULL	NULL	0	NULL	fingers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Force-stabilization by all eight fingers improved quantitatively with practice .
	manualset3
245726	4	428006	16	NULL	NULL	0	NULL	practice	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Force-stabilization by all eight fingers improved quantitatively with practice .
	manualset3
245727	1	428007	16	NULL	NULL	NULL	NULL	Force production	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Force production was recorded , and intracellular concentrations of phosphorus compounds and pH were measured in the flexor digitorum profundus of the active forearm .
	manualset3
245728	2	428007	16	NULL	NULL	0	NULL	intracellular concentrations	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Force production was recorded , and intracellular concentrations of phosphorus compounds and pH were measured in the flexor digitorum profundus of the active forearm .
	manualset3
245729	3	428007	16	NULL	NULL	0	NULL	 phosphorus compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Force production was recorded , and intracellular concentrations of phosphorus compounds and pH were measured in the flexor digitorum profundus of the active forearm .
	manualset3
245730	4	428007	16	NULL	NULL	0	NULL	pH	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Force production was recorded , and intracellular concentrations of phosphorus compounds and pH were measured in the flexor digitorum profundus of the active forearm .
	manualset3
245731	5	428007	16	NULL	NULL	0	NULL	flexor digitorum profundus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Force production was recorded , and intracellular concentrations of phosphorus compounds and pH were measured in the flexor digitorum profundus of the active forearm .
	manualset3
245732	6	428007	16	NULL	NULL	0	NULL	forearm	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Force production was recorded , and intracellular concentrations of phosphorus compounds and pH were measured in the flexor digitorum profundus of the active forearm .
	manualset3
245733	1	428008	16	NULL	NULL	NULL	NULL	Forced expiratory volume ( FEV1	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Forced expiratory volume ( FEV1 ; percentage predicted ) , determined as an indicator of lung injury in CF , was evaluated as an immunologic response to pseudomonas , against a profile derived from combined serial data on both the circulating immune complexes ( CIC ) and the Ps .
	manualset3
245734	2	428008	16	NULL	NULL	0	NULL	percentage predicted	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Forced expiratory volume ( FEV1 ; percentage predicted ) , determined as an indicator of lung injury in CF , was evaluated as an immunologic response to pseudomonas , against a profile derived from combined serial data on both the circulating immune complexes ( CIC ) and the Ps .
	manualset3
245735	3	428008	16	NULL	NULL	NULL	NULL	indicator of lung injury	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Forced expiratory volume ( FEV1 ; percentage predicted ) , determined as an indicator of lung injury in CF , was evaluated as an immunologic response to pseudomonas , against a profile derived from combined serial data on both the circulating immune complexes ( CIC ) and the Ps .
	manualset3
245737	5	428008	16	NULL	NULL	0	NULL	CF	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Forced expiratory volume ( FEV1 ; percentage predicted ) , determined as an indicator of lung injury in CF , was evaluated as an immunologic response to pseudomonas , against a profile derived from combined serial data on both the circulating immune complexes ( CIC ) and the Ps .
	manualset3
245738	6	428008	16	NULL	NULL	0	NULL	immunologic response	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Forced expiratory volume ( FEV1 ; percentage predicted ) , determined as an indicator of lung injury in CF , was evaluated as an immunologic response to pseudomonas , against a profile derived from combined serial data on both the circulating immune complexes ( CIC ) and the Ps .
	manualset3
245739	7	428008	16	NULL	NULL	0	NULL	pseudomonas	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Forced expiratory volume ( FEV1 ; percentage predicted ) , determined as an indicator of lung injury in CF , was evaluated as an immunologic response to pseudomonas , against a profile derived from combined serial data on both the circulating immune complexes ( CIC ) and the Ps .
	manualset3
245740	8	428008	16	NULL	NULL	0	NULL	profile	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Forced expiratory volume ( FEV1 ; percentage predicted ) , determined as an indicator of lung injury in CF , was evaluated as an immunologic response to pseudomonas , against a profile derived from combined serial data on both the circulating immune complexes ( CIC ) and the Ps .
	manualset3
245741	9	428008	16	NULL	NULL	0	NULL	combined serial data	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Forced expiratory volume ( FEV1 ; percentage predicted ) , determined as an indicator of lung injury in CF , was evaluated as an immunologic response to pseudomonas , against a profile derived from combined serial data on both the circulating immune complexes ( CIC ) and the Ps .
	manualset3
245742	10	428008	16	NULL	NULL	0	NULL	circulating immune complexes ( CIC )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Forced expiratory volume ( FEV1 ; percentage predicted ) , determined as an indicator of lung injury in CF , was evaluated as an immunologic response to pseudomonas , against a profile derived from combined serial data on both the circulating immune complexes ( CIC ) and the Ps .
	manualset3
245743	11	428008	16	NULL	NULL	0	NULL	Ps	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Forced expiratory volume ( FEV1 ; percentage predicted ) , determined as an indicator of lung injury in CF , was evaluated as an immunologic response to pseudomonas , against a profile derived from combined serial data on both the circulating immune complexes ( CIC ) and the Ps .
	manualset3
245744	1	428009	16	NULL	NULL	0	NULL	Forced transcription	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Forced transcription of xisF in vegetative cells did not result in excision of the fdxN element , suggesting that other factors may be involved in cell-type specificity .
	manualset3
245745	2	428009	16	NULL	NULL	0	NULL	xisF	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Forced transcription of xisF in vegetative cells did not result in excision of the fdxN element , suggesting that other factors may be involved in cell-type specificity .
	manualset3
245746	3	428009	16	NULL	NULL	NULL	NULL	vegetative cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Forced transcription of xisF in vegetative cells did not result in excision of the fdxN element , suggesting that other factors may be involved in cell-type specificity .
	manualset3
245747	4	428009	16	NULL	NULL	0	NULL	excision	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Forced transcription of xisF in vegetative cells did not result in excision of the fdxN element , suggesting that other factors may be involved in cell-type specificity .
	manualset3
245748	5	428009	16	NULL	NULL	0	NULL	fdxN element	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Forced transcription of xisF in vegetative cells did not result in excision of the fdxN element , suggesting that other factors may be involved in cell-type specificity .
	manualset3
245749	6	428009	16	NULL	NULL	0	NULL	factors	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Forced transcription of xisF in vegetative cells did not result in excision of the fdxN element , suggesting that other factors may be involved in cell-type specificity .
	manualset3
245750	7	428009	16	NULL	NULL	0	NULL	cell-type specificity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Forced transcription of xisF in vegetative cells did not result in excision of the fdxN element , suggesting that other factors may be involved in cell-type specificity .
	manualset3
245751	1	428010	16	NULL	NULL	0	NULL	Forearm blood flow	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Forearm blood flow and sweating also showed time-of-day differences , but these did not co-vary with rectal temperature .
	manualset3
245752	2	428010	16	NULL	NULL	0	NULL	sweating	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Forearm blood flow and sweating also showed time-of-day differences , but these did not co-vary with rectal temperature .
	manualset3
245753	3	428010	16	NULL	NULL	NULL	NULL	time-of-day differences	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Forearm blood flow and sweating also showed time-of-day differences , but these did not co-vary with rectal temperature .
	manualset3
245754	4	428010	16	NULL	NULL	0	NULL	rectal temperature	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Forearm blood flow and sweating also showed time-of-day differences , but these did not co-vary with rectal temperature .
	manualset3
245755	1	428011	16	NULL	NULL	0	NULL	Forearm venous blood	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Forearm venous blood demonstrated a rise in hydrogen ion concentration and a fall in oxygen tension during venous occlusion , which may contribute to the vasodilatation phase .
	manualset3
245756	2	428011	16	NULL	NULL	0	NULL	rise	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Forearm venous blood demonstrated a rise in hydrogen ion concentration and a fall in oxygen tension during venous occlusion , which may contribute to the vasodilatation phase .
	manualset3
245757	3	428011	16	NULL	NULL	NULL	NULL	hydrogen ion concentration	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Forearm venous blood demonstrated a rise in hydrogen ion concentration and a fall in oxygen tension during venous occlusion , which may contribute to the vasodilatation phase .
	manualset3
245759	5	428011	16	NULL	NULL	0	NULL	fall	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Forearm venous blood demonstrated a rise in hydrogen ion concentration and a fall in oxygen tension during venous occlusion , which may contribute to the vasodilatation phase .
	manualset3
245760	6	428011	16	NULL	NULL	0	NULL	oxygen tension	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Forearm venous blood demonstrated a rise in hydrogen ion concentration and a fall in oxygen tension during venous occlusion , which may contribute to the vasodilatation phase .
	manualset3
245761	7	428011	16	NULL	NULL	0	NULL	venous occlusion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Forearm venous blood demonstrated a rise in hydrogen ion concentration and a fall in oxygen tension during venous occlusion , which may contribute to the vasodilatation phase .
	manualset3
245762	8	428011	16	NULL	NULL	0	NULL	vasodilatation phase	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Forearm venous blood demonstrated a rise in hydrogen ion concentration and a fall in oxygen tension during venous occlusion , which may contribute to the vasodilatation phase .
	manualset3
245763	1	428012	16	NULL	NULL	0	NULL	Forebrain	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Forebrain NR2B overexpression facilitating the prefrontal cortex long-term potentiation and enhancing working memory function in mice .
	manualset3
245764	2	428012	16	NULL	NULL	0	NULL	NR2B overexpression	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Forebrain NR2B overexpression facilitating the prefrontal cortex long-term potentiation and enhancing working memory function in mice .
	manualset3
245765	3	428012	16	NULL	NULL	0	NULL	prefrontal cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Forebrain NR2B overexpression facilitating the prefrontal cortex long-term potentiation and enhancing working memory function in mice .
	manualset3
245766	4	428012	16	NULL	NULL	0	NULL	long-term potentiation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Forebrain NR2B overexpression facilitating the prefrontal cortex long-term potentiation and enhancing working memory function in mice .
	manualset3
245767	5	428012	16	NULL	NULL	0	NULL	working memory function	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Forebrain NR2B overexpression facilitating the prefrontal cortex long-term potentiation and enhancing working memory function in mice .
	manualset3
245768	6	428012	16	NULL	NULL	0	NULL	mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Forebrain NR2B overexpression facilitating the prefrontal cortex long-term potentiation and enhancing working memory function in mice .
	manualset3
245769	1	428013	16	NULL	NULL	0	NULL	Forebrain limbic sites	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Forebrain limbic sites connect with the PVN via interactions with GABA-containing neurons in the bed nucleus of the stria terminalis , preoptic area and hypothalamus .
	manualset3
245770	2	428013	16	NULL	NULL	0	NULL	PVN	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Forebrain limbic sites connect with the PVN via interactions with GABA-containing neurons in the bed nucleus of the stria terminalis , preoptic area and hypothalamus .
	manualset3
245771	3	428013	16	NULL	NULL	NULL	NULL	interactions	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Forebrain limbic sites connect with the PVN via interactions with GABA-containing neurons in the bed nucleus of the stria terminalis , preoptic area and hypothalamus .
	manualset3
245772	4	428013	16	NULL	NULL	0	NULL	GABA-containing neurons	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Forebrain limbic sites connect with the PVN via interactions with GABA-containing neurons in the bed nucleus of the stria terminalis , preoptic area and hypothalamus .
	manualset3
245773	5	428013	16	NULL	NULL	0	NULL	bed nucleus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Forebrain limbic sites connect with the PVN via interactions with GABA-containing neurons in the bed nucleus of the stria terminalis , preoptic area and hypothalamus .
	manualset3
245774	6	428013	16	NULL	NULL	0	NULL	stria terminalis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Forebrain limbic sites connect with the PVN via interactions with GABA-containing neurons in the bed nucleus of the stria terminalis , preoptic area and hypothalamus .
	manualset3
245775	7	428013	16	NULL	NULL	0	NULL	preoptic area	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Forebrain limbic sites connect with the PVN via interactions with GABA-containing neurons in the bed nucleus of the stria terminalis , preoptic area and hypothalamus .
	manualset3
245776	8	428013	16	NULL	NULL	0	NULL	hypothalamus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Forebrain limbic sites connect with the PVN via interactions with GABA-containing neurons in the bed nucleus of the stria terminalis , preoptic area and hypothalamus .
	manualset3
245777	1	428014	16	NULL	NULL	0	NULL	Forensic art	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Forensic art : a police artist 's experience .
	manualset3
245778	2	428014	16	NULL	NULL	0	NULL	police artist	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Forensic art : a police artist 's experience .
	manualset3
245779	3	428014	16	NULL	NULL	0	NULL	experience	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Forensic art : a police artist 's experience .
	manualset3
245784	1	428015	16	NULL	NULL	0	NULL	JEM spotlight	Journal												NULL		0	NULL	NULL	NULL	NULL	NULL	Foreword : JEM spotlight : Nuclear desalination -- environmental impacts and implications for planning and monitoring activities .
	manualset3
245785	2	428015	16	NULL	NULL	0	NULL	Nuclear desalination	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Foreword : JEM spotlight : Nuclear desalination -- environmental impacts and implications for planning and monitoring activities .
	manualset3
245868	3	428015	16	NULL	NULL	0	NULL	environmental impacts	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Foreword : JEM spotlight : Nuclear desalination -- environmental impacts and implications for planning and monitoring activities .
	manualset3
245869	4	428015	16	NULL	NULL	NULL	NULL	implications	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Foreword : JEM spotlight : Nuclear desalination -- environmental impacts and implications for planning and monitoring activities .
	manualset3
245870	5	428015	16	NULL	NULL	0	NULL	planning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Foreword : JEM spotlight : Nuclear desalination -- environmental impacts and implications for planning and monitoring activities .
	manualset3
245871	6	428015	16	NULL	NULL	0	NULL	monitoring activities	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Foreword : JEM spotlight : Nuclear desalination -- environmental impacts and implications for planning and monitoring activities .
	manualset3
245786	1	428016	16	NULL	NULL	0	NULL	Formaldehyde	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Formaldehyde is a widely used irritating chemical , mainly employed as disinfectant or in the production of multiple resin products employed in the wood , shoe , and clothing industries .
	manualset3
245787	2	428016	16	NULL	NULL	0	NULL	chemical	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Formaldehyde is a widely used irritating chemical , mainly employed as disinfectant or in the production of multiple resin products employed in the wood , shoe , and clothing industries .
	manualset3
245788	3	428016	16	NULL	NULL	0	NULL	disinfectant	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Formaldehyde is a widely used irritating chemical , mainly employed as disinfectant or in the production of multiple resin products employed in the wood , shoe , and clothing industries .
	manualset3
245789	4	428016	16	NULL	NULL	0	NULL	production	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Formaldehyde is a widely used irritating chemical , mainly employed as disinfectant or in the production of multiple resin products employed in the wood , shoe , and clothing industries .
	manualset3
245790	5	428016	16	NULL	NULL	NULL	NULL	resin products	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Formaldehyde is a widely used irritating chemical , mainly employed as disinfectant or in the production of multiple resin products employed in the wood , shoe , and clothing industries .
	manualset3
245791	6	428016	16	NULL	NULL	0	NULL	wood industries	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Formaldehyde is a widely used irritating chemical , mainly employed as disinfectant or in the production of multiple resin products employed in the wood , shoe , and clothing industries .
	manualset3
245792	7	428016	16	NULL	NULL	0	NULL	shoe industries	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Formaldehyde is a widely used irritating chemical , mainly employed as disinfectant or in the production of multiple resin products employed in the wood , shoe , and clothing industries .
	manualset3
245793	8	428016	16	NULL	NULL	0	NULL	clothing industries	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Formaldehyde is a widely used irritating chemical , mainly employed as disinfectant or in the production of multiple resin products employed in the wood , shoe , and clothing industries .
	manualset3
245794	1	428017	16	NULL	NULL	0	NULL	Formate dehydrogenases ( FDHs )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Formate dehydrogenases ( FDHs ) are enzymes that catalyze the formate oxidation to carbon dioxide and that contain either Mo or W in a mononuclear form in the active site .
	manualset3
245795	2	428017	16	NULL	NULL	0	NULL	enzymes	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Formate dehydrogenases ( FDHs ) are enzymes that catalyze the formate oxidation to carbon dioxide and that contain either Mo or W in a mononuclear form in the active site .
	manualset3
245796	3	428017	16	NULL	NULL	0	NULL	formate oxidation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Formate dehydrogenases ( FDHs ) are enzymes that catalyze the formate oxidation to carbon dioxide and that contain either Mo or W in a mononuclear form in the active site .
	manualset3
245797	4	428017	16	NULL	NULL	0	NULL	carbon dioxide	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Formate dehydrogenases ( FDHs ) are enzymes that catalyze the formate oxidation to carbon dioxide and that contain either Mo or W in a mononuclear form in the active site .
	manualset3
245798	5	428017	16	NULL	NULL	0	NULL	Mo	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Formate dehydrogenases ( FDHs ) are enzymes that catalyze the formate oxidation to carbon dioxide and that contain either Mo or W in a mononuclear form in the active site .
	manualset3
245799	6	428017	16	NULL	NULL	0	NULL	W	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Formate dehydrogenases ( FDHs ) are enzymes that catalyze the formate oxidation to carbon dioxide and that contain either Mo or W in a mononuclear form in the active site .
	manualset3
245800	7	428017	16	NULL	NULL	NULL	NULL	mononuclear form	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Formate dehydrogenases ( FDHs ) are enzymes that catalyze the formate oxidation to carbon dioxide and that contain either Mo or W in a mononuclear form in the active site .
	manualset3
245801	8	428017	16	NULL	NULL	0	NULL	active site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Formate dehydrogenases ( FDHs ) are enzymes that catalyze the formate oxidation to carbon dioxide and that contain either Mo or W in a mononuclear form in the active site .
	manualset3
245802	1	428018	16	NULL	NULL	NULL	NULL	Formation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Formation of STAT5/PPARgamma transcriptional complex modulates angiogenic cell bioavailability in diabetes .
	manualset3
245803	2	428018	16	NULL	NULL	0	NULL	 STAT5/PPARgamma transcriptional complex	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Formation of STAT5/PPARgamma transcriptional complex modulates angiogenic cell bioavailability in diabetes .
	manualset3
245804	3	428018	16	NULL	NULL	0	NULL	angiogenic cell bioavailability	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Formation of STAT5/PPARgamma transcriptional complex modulates angiogenic cell bioavailability in diabetes .
	manualset3
245805	4	428018	16	NULL	NULL	0	NULL	diabetes	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Formation of STAT5/PPARgamma transcriptional complex modulates angiogenic cell bioavailability in diabetes .
	manualset3
245806	1	428019	16	NULL	NULL	0	NULL	Formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Formation of nontoxic reactive metabolites of p-bromophenol .
	manualset3
245807	2	428019	16	NULL	NULL	0	NULL	nontoxic reactive metabolites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Formation of nontoxic reactive metabolites of p-bromophenol .
	manualset3
245808	3	428019	16	NULL	NULL	0	NULL	p-bromophenol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Formation of nontoxic reactive metabolites of p-bromophenol .
	manualset3
245809	1	428020	16	NULL	NULL	0	NULL	Formation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Formation of serum amyloid protein-rich subfractions .
	manualset3
245810	2	428020	16	NULL	NULL	0	NULL	serum amyloid protein-rich subfractions	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Formation of serum amyloid protein-rich subfractions .
	manualset3
245811	1	428021	16	NULL	NULL	0	NULL	evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Formative evaluation of an intervention to increase compliance to HIV therapies : the ALP project .
	manualset3
245812	2	428021	16	NULL	NULL	0	NULL	intervention	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Formative evaluation of an intervention to increase compliance to HIV therapies : the ALP project .
	manualset3
245813	3	428021	16	NULL	NULL	0	NULL	compliance	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Formative evaluation of an intervention to increase compliance to HIV therapies : the ALP project .
	manualset3
245814	4	428021	16	NULL	NULL	0	NULL	HIV therapies	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Formative evaluation of an intervention to increase compliance to HIV therapies : the ALP project .
	manualset3
245815	5	428021	16	NULL	NULL	NULL	NULL	ALP project	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Formative evaluation of an intervention to increase compliance to HIV therapies : the ALP project .
	manualset3
245816	1	428022	16	NULL	NULL	0	NULL	result	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Formed as a result of slow , spontaneous and non-enzymatic glycation reactions , Hb-AGE possesses a characteristic autofluorescence at 308/345 nm ( lambda ( ex ) / lambda ( em ) ) .
	manualset3
245817	2	428022	16	NULL	NULL	0	NULL	non-enzymatic glycation reactions	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Formed as a result of slow , spontaneous and non-enzymatic glycation reactions , Hb-AGE possesses a characteristic autofluorescence at 308/345 nm ( lambda ( ex ) / lambda ( em ) ) .
	manualset3
245818	3	428022	16	NULL	NULL	0	NULL	Hb-AGE	GeneOrProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Formed as a result of slow , spontaneous and non-enzymatic glycation reactions , Hb-AGE possesses a characteristic autofluorescence at 308/345 nm ( lambda ( ex ) / lambda ( em ) ) .
	manualset3
245819	4	428022	16	NULL	NULL	0	NULL	autofluorescence	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Formed as a result of slow , spontaneous and non-enzymatic glycation reactions , Hb-AGE possesses a characteristic autofluorescence at 308/345 nm ( lambda ( ex ) / lambda ( em ) ) .
	manualset3
245820	5	428022	16	NULL	NULL	0	NULL	308/345 nm ( lambda ( ex ) / lambda ( em ) )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Formed as a result of slow , spontaneous and non-enzymatic glycation reactions , Hb-AGE possesses a characteristic autofluorescence at 308/345 nm ( lambda ( ex ) / lambda ( em ) ) .
	manualset3
245821	1	428023	16	NULL	NULL	0	NULL	Former hand territory activity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Former hand territory activity increases after amputation during intact hand movements , but is unaffected by illusory visual feedback .
	manualset3
245822	2	428023	16	NULL	NULL	0	NULL	amputation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Former hand territory activity increases after amputation during intact hand movements , but is unaffected by illusory visual feedback .
	manualset3
245823	3	428023	16	NULL	NULL	0	NULL	intact hand movements	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Former hand territory activity increases after amputation during intact hand movements , but is unaffected by illusory visual feedback .
	manualset3
245824	4	428023	16	NULL	NULL	0	NULL	illusory visual feedback	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Former hand territory activity increases after amputation during intact hand movements , but is unaffected by illusory visual feedback .
	manualset3
245825	1	428024	16	NULL	NULL	0	NULL	Formulations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Formulations and clinical management , mechanisms of action , noncontraceptive benefits of use , therapeutic uses in addition to contraception , side effects , contraindications to use , and drug-drug interactions are described .
	manualset3
245826	2	428024	16	NULL	NULL	0	NULL	clinical management	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Formulations and clinical management , mechanisms of action , noncontraceptive benefits of use , therapeutic uses in addition to contraception , side effects , contraindications to use , and drug-drug interactions are described .
	manualset3
245827	3	428024	16	NULL	NULL	0	NULL	noncontraceptive benefits of use	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Formulations and clinical management , mechanisms of action , noncontraceptive benefits of use , therapeutic uses in addition to contraception , side effects , contraindications to use , and drug-drug interactions are described .
	manualset3
245828	4	428024	16	NULL	NULL	0	NULL	therapeutic uses	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Formulations and clinical management , mechanisms of action , noncontraceptive benefits of use , therapeutic uses in addition to contraception , side effects , contraindications to use , and drug-drug interactions are described .
	manualset3
245829	5	428024	16	NULL	NULL	0	NULL	addition	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Formulations and clinical management , mechanisms of action , noncontraceptive benefits of use , therapeutic uses in addition to contraception , side effects , contraindications to use , and drug-drug interactions are described .
	manualset3
245830	6	428024	16	NULL	NULL	0	NULL	contraception	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Formulations and clinical management , mechanisms of action , noncontraceptive benefits of use , therapeutic uses in addition to contraception , side effects , contraindications to use , and drug-drug interactions are described .
	manualset3
245831	7	428024	16	NULL	NULL	0	NULL	side effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Formulations and clinical management , mechanisms of action , noncontraceptive benefits of use , therapeutic uses in addition to contraception , side effects , contraindications to use , and drug-drug interactions are described .
	manualset3
245832	8	428024	16	NULL	NULL	0	NULL	contraindications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Formulations and clinical management , mechanisms of action , noncontraceptive benefits of use , therapeutic uses in addition to contraception , side effects , contraindications to use , and drug-drug interactions are described .
	manualset3
245833	9	428024	16	NULL	NULL	0	NULL	drug-drug interactions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Formulations and clinical management , mechanisms of action , noncontraceptive benefits of use , therapeutic uses in addition to contraception , side effects , contraindications to use , and drug-drug interactions are described .
	manualset3
247064	10	428024	16	NULL	NULL	0	NULL	mechanisms of action	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Formulations and clinical management , mechanisms of action , noncontraceptive benefits of use , therapeutic uses in addition to contraception , side effects , contraindications to use , and drug-drug interactions are described .
	manualset3
245834	1	428025	16	NULL	NULL	0	NULL	Forskolin-stimulated adenylate cyclase ( FSAC ) activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Forskolin-stimulated adenylate cyclase ( FSAC ) activity was used as a model to elucidate the effect of SPD on D2 receptors .
	manualset3
245835	2	428025	16	NULL	NULL	0	NULL	model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Forskolin-stimulated adenylate cyclase ( FSAC ) activity was used as a model to elucidate the effect of SPD on D2 receptors .
	manualset3
245836	3	428025	16	NULL	NULL	0	NULL	effect	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Forskolin-stimulated adenylate cyclase ( FSAC ) activity was used as a model to elucidate the effect of SPD on D2 receptors .
	manualset3
245837	4	428025	16	NULL	NULL	0	NULL	SPD	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Forskolin-stimulated adenylate cyclase ( FSAC ) activity was used as a model to elucidate the effect of SPD on D2 receptors .
	manualset3
245838	5	428025	16	NULL	NULL	0	NULL	D2 receptors	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Forskolin-stimulated adenylate cyclase ( FSAC ) activity was used as a model to elucidate the effect of SPD on D2 receptors .
	manualset3
245839	1	428026	16	NULL	NULL	0	NULL	Forskolin	SmallMolecule												NULL		0	NULL	NULL	NULL	NULL	NULL	Forskolin increased the phosphorylation of Ser40 in hTH1 and Ser44 in hTH2 .
	manualset3
245840	2	428026	16	NULL	NULL	0	NULL	phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Forskolin increased the phosphorylation of Ser40 in hTH1 and Ser44 in hTH2 .
	manualset3
245841	3	428026	16	NULL	NULL	0	NULL	Ser40	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Forskolin increased the phosphorylation of Ser40 in hTH1 and Ser44 in hTH2 .
	manualset3
245842	4	428026	16	NULL	NULL	0	NULL	hTH1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Forskolin increased the phosphorylation of Ser40 in hTH1 and Ser44 in hTH2 .
	manualset3
245843	5	428026	16	NULL	NULL	0	NULL	Ser44	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Forskolin increased the phosphorylation of Ser40 in hTH1 and Ser44 in hTH2 .
	manualset3
245844	6	428026	16	NULL	NULL	0	NULL	hTH2	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Forskolin increased the phosphorylation of Ser40 in hTH1 and Ser44 in hTH2 .
	manualset3
245845	1	428027	16	NULL	NULL	0	NULL	Forty-eight	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-eight of the masses had a signal intensity similar to that of muscle in T1-weighted images and higher than , equal to or lower than that of fat in T2-weighted images .
	manualset3
245846	2	428027	16	NULL	NULL	NULL	NULL	masses	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Forty-eight of the masses had a signal intensity similar to that of muscle in T1-weighted images and higher than , equal to or lower than that of fat in T2-weighted images .
	manualset3
245847	3	428027	16	NULL	NULL	0	NULL	signal intensity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-eight of the masses had a signal intensity similar to that of muscle in T1-weighted images and higher than , equal to or lower than that of fat in T2-weighted images .
	manualset3
245848	4	428027	16	NULL	NULL	0	NULL	muscle	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-eight of the masses had a signal intensity similar to that of muscle in T1-weighted images and higher than , equal to or lower than that of fat in T2-weighted images .
	manualset3
245849	5	428027	16	NULL	NULL	0	NULL	T1-weighted images	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-eight of the masses had a signal intensity similar to that of muscle in T1-weighted images and higher than , equal to or lower than that of fat in T2-weighted images .
	manualset3
245850	6	428027	16	NULL	NULL	0	NULL	fat	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-eight of the masses had a signal intensity similar to that of muscle in T1-weighted images and higher than , equal to or lower than that of fat in T2-weighted images .
	manualset3
245851	7	428027	16	NULL	NULL	0	NULL	T2-weighted images	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-eight of the masses had a signal intensity similar to that of muscle in T1-weighted images and higher than , equal to or lower than that of fat in T2-weighted images .
	manualset3
245852	1	428028	16	NULL	NULL	0	NULL	Research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Research on the behavior of the C-reactive protein in pulmonary tuberculosis ) .
	manualset3
245853	2	428028	16	NULL	NULL	0	NULL	behavior	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Research on the behavior of the C-reactive protein in pulmonary tuberculosis ) .
	manualset3
245854	3	428028	16	NULL	NULL	0	NULL	C-reactive protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	( Research on the behavior of the C-reactive protein in pulmonary tuberculosis ) .
	manualset3
245855	4	428028	16	NULL	NULL	0	NULL	pulmonary tuberculosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Research on the behavior of the C-reactive protein in pulmonary tuberculosis ) .
	manualset3
245856	1	428029	16	NULL	NULL	0	NULL	Forty-five	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-five of seventy-one regenerating neurites ( 64 % ) grew beyond the level of the hemisection .
	manualset3
245857	2	428029	16	NULL	NULL	0	NULL	seventy-one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-five of seventy-one regenerating neurites ( 64 % ) grew beyond the level of the hemisection .
	manualset3
245858	3	428029	16	NULL	NULL	0	NULL	regenerating neurites	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-five of seventy-one regenerating neurites ( 64 % ) grew beyond the level of the hemisection .
	manualset3
245859	4	428029	16	NULL	NULL	0	NULL	64 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-five of seventy-one regenerating neurites ( 64 % ) grew beyond the level of the hemisection .
	manualset3
245860	5	428029	16	NULL	NULL	0	NULL	level	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-five of seventy-one regenerating neurites ( 64 % ) grew beyond the level of the hemisection .
	manualset3
245861	6	428029	16	NULL	NULL	0	NULL	hemisection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-five of seventy-one regenerating neurites ( 64 % ) grew beyond the level of the hemisection .
	manualset3
245862	1	428030	16	NULL	NULL	0	NULL	Forty-four patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-four patients ( 21 men and 23 women ) were assessed at admission and before discharge with the Functional Independence Measure ( FIM ) .
	manualset3
245863	2	428030	16	NULL	NULL	0	NULL	21 men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-four patients ( 21 men and 23 women ) were assessed at admission and before discharge with the Functional Independence Measure ( FIM ) .
	manualset3
245864	3	428030	16	NULL	NULL	0	NULL	23 women	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-four patients ( 21 men and 23 women ) were assessed at admission and before discharge with the Functional Independence Measure ( FIM ) .
	manualset3
245865	4	428030	16	NULL	NULL	0	NULL	admission	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-four patients ( 21 men and 23 women ) were assessed at admission and before discharge with the Functional Independence Measure ( FIM ) .
	manualset3
245866	5	428030	16	NULL	NULL	0	NULL	discharge	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-four patients ( 21 men and 23 women ) were assessed at admission and before discharge with the Functional Independence Measure ( FIM ) .
	manualset3
245867	6	428030	16	NULL	NULL	0	NULL	Functional Independence Measure ( FIM )	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-four patients ( 21 men and 23 women ) were assessed at admission and before discharge with the Functional Independence Measure ( FIM ) .
	manualset3
230712	1	428031	15	NULL	NULL	0	NULL	Forty-four percent	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-four percent of the patients experienced at least one severe hypoglycemic episode ( need for assistance ( grade III ) , loss of consciousness with or without convulsions ( grade IV ) ) during the survey period .
	manualset3
230713	2	428031	15	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-four percent of the patients experienced at least one severe hypoglycemic episode ( need for assistance ( grade III ) , loss of consciousness with or without convulsions ( grade IV ) ) during the survey period .
	manualset3
230714	3	428031	15	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-four percent of the patients experienced at least one severe hypoglycemic episode ( need for assistance ( grade III ) , loss of consciousness with or without convulsions ( grade IV ) ) during the survey period .
	manualset3
230715	4	428031	15	NULL	NULL	0	NULL	hypoglycemic episode	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-four percent of the patients experienced at least one severe hypoglycemic episode ( need for assistance ( grade III ) , loss of consciousness with or without convulsions ( grade IV ) ) during the survey period .
	manualset3
230716	5	428031	15	NULL	NULL	0	NULL	need for assistance ( grade III )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-four percent of the patients experienced at least one severe hypoglycemic episode ( need for assistance ( grade III ) , loss of consciousness with or without convulsions ( grade IV ) ) during the survey period .
	manualset3
230717	6	428031	15	NULL	NULL	0	NULL	loss of consciousness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-four percent of the patients experienced at least one severe hypoglycemic episode ( need for assistance ( grade III ) , loss of consciousness with or without convulsions ( grade IV ) ) during the survey period .
	manualset3
230718	7	428031	15	NULL	NULL	0	NULL	convulsions ( grade IV )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-four percent of the patients experienced at least one severe hypoglycemic episode ( need for assistance ( grade III ) , loss of consciousness with or without convulsions ( grade IV ) ) during the survey period .
	manualset3
230719	8	428031	15	NULL	NULL	0	NULL	survey period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-four percent of the patients experienced at least one severe hypoglycemic episode ( need for assistance ( grade III ) , loss of consciousness with or without convulsions ( grade IV ) ) during the survey period .
	manualset3
230720	1	428032	15	NULL	NULL	0	NULL	Forty-one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-one aroma-active compounds were observed in unpasteurized single strength juice , whereas 27 components were found in the unflavored reconstituted concentrate .
	manualset3
230721	2	428032	15	NULL	NULL	0	NULL	aroma-active compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-one aroma-active compounds were observed in unpasteurized single strength juice , whereas 27 components were found in the unflavored reconstituted concentrate .
	manualset3
230722	3	428032	15	NULL	NULL	NULL	NULL	single strength juice	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Forty-one aroma-active compounds were observed in unpasteurized single strength juice , whereas 27 components were found in the unflavored reconstituted concentrate .
	manualset3
230723	4	428032	15	NULL	NULL	0	NULL	27 components	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-one aroma-active compounds were observed in unpasteurized single strength juice , whereas 27 components were found in the unflavored reconstituted concentrate .
	manualset3
230724	5	428032	15	NULL	NULL	NULL	NULL	reconstituted concentrate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Forty-one aroma-active compounds were observed in unpasteurized single strength juice , whereas 27 components were found in the unflavored reconstituted concentrate .
	manualset3
230725	1	428033	15	NULL	NULL	0	NULL	Forty-seven	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-seven adult orthodontic patients with fixed orthodontic appliances were divided into three study groups : ( 1 ) oral irrigation with automatic toothbrush , ( n = 16 ) ; ( 2 ) oral irrigation with manual toothbrushing , ( n = 16 ) ; ( 3 ) control group with continued normal toothbrushing only , ( n = 15 ) .
	manualset3
230726	2	428033	15	NULL	NULL	0	NULL	adult orthodontic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-seven adult orthodontic patients with fixed orthodontic appliances were divided into three study groups : ( 1 ) oral irrigation with automatic toothbrush , ( n = 16 ) ; ( 2 ) oral irrigation with manual toothbrushing , ( n = 16 ) ; ( 3 ) control group with continued normal toothbrushing only , ( n = 15 ) .
	manualset3
230727	3	428033	15	NULL	NULL	0	NULL	orthodontic appliances	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-seven adult orthodontic patients with fixed orthodontic appliances were divided into three study groups : ( 1 ) oral irrigation with automatic toothbrush , ( n = 16 ) ; ( 2 ) oral irrigation with manual toothbrushing , ( n = 16 ) ; ( 3 ) control group with continued normal toothbrushing only , ( n = 15 ) .
	manualset3
230728	4	428033	15	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-seven adult orthodontic patients with fixed orthodontic appliances were divided into three study groups : ( 1 ) oral irrigation with automatic toothbrush , ( n = 16 ) ; ( 2 ) oral irrigation with manual toothbrushing , ( n = 16 ) ; ( 3 ) control group with continued normal toothbrushing only , ( n = 15 ) .
	manualset3
230729	5	428033	15	NULL	NULL	0	NULL	study groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-seven adult orthodontic patients with fixed orthodontic appliances were divided into three study groups : ( 1 ) oral irrigation with automatic toothbrush , ( n = 16 ) ; ( 2 ) oral irrigation with manual toothbrushing , ( n = 16 ) ; ( 3 ) control group with continued normal toothbrushing only , ( n = 15 ) .
	manualset3
230730	6	428033	15	NULL	NULL	0	NULL	oral irrigation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-seven adult orthodontic patients with fixed orthodontic appliances were divided into three study groups : ( 1 ) oral irrigation with automatic toothbrush , ( n = 16 ) ; ( 2 ) oral irrigation with manual toothbrushing , ( n = 16 ) ; ( 3 ) control group with continued normal toothbrushing only , ( n = 15 ) .
	manualset3
230731	7	428033	15	NULL	NULL	0	NULL	automatic toothbrush	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-seven adult orthodontic patients with fixed orthodontic appliances were divided into three study groups : ( 1 ) oral irrigation with automatic toothbrush , ( n = 16 ) ; ( 2 ) oral irrigation with manual toothbrushing , ( n = 16 ) ; ( 3 ) control group with continued normal toothbrushing only , ( n = 15 ) .
	manualset3
230732	8	428033	15	NULL	NULL	0	NULL	 n = 16	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-seven adult orthodontic patients with fixed orthodontic appliances were divided into three study groups : ( 1 ) oral irrigation with automatic toothbrush , ( n = 16 ) ; ( 2 ) oral irrigation with manual toothbrushing , ( n = 16 ) ; ( 3 ) control group with continued normal toothbrushing only , ( n = 15 ) .
	manualset3
230733	9	428033	15	NULL	NULL	0	NULL	oral irrigation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-seven adult orthodontic patients with fixed orthodontic appliances were divided into three study groups : ( 1 ) oral irrigation with automatic toothbrush , ( n = 16 ) ; ( 2 ) oral irrigation with manual toothbrushing , ( n = 16 ) ; ( 3 ) control group with continued normal toothbrushing only , ( n = 15 ) .
	manualset3
230734	10	428033	15	NULL	NULL	0	NULL	manual toothbrushing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-seven adult orthodontic patients with fixed orthodontic appliances were divided into three study groups : ( 1 ) oral irrigation with automatic toothbrush , ( n = 16 ) ; ( 2 ) oral irrigation with manual toothbrushing , ( n = 16 ) ; ( 3 ) control group with continued normal toothbrushing only , ( n = 15 ) .
	manualset3
230735	11	428033	15	NULL	NULL	0	NULL	n = 16	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-seven adult orthodontic patients with fixed orthodontic appliances were divided into three study groups : ( 1 ) oral irrigation with automatic toothbrush , ( n = 16 ) ; ( 2 ) oral irrigation with manual toothbrushing , ( n = 16 ) ; ( 3 ) control group with continued normal toothbrushing only , ( n = 15 ) .
	manualset3
230736	12	428033	15	NULL	NULL	0	NULL	control group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-seven adult orthodontic patients with fixed orthodontic appliances were divided into three study groups : ( 1 ) oral irrigation with automatic toothbrush , ( n = 16 ) ; ( 2 ) oral irrigation with manual toothbrushing , ( n = 16 ) ; ( 3 ) control group with continued normal toothbrushing only , ( n = 15 ) .
	manualset3
230737	13	428033	15	NULL	NULL	0	NULL	normal toothbrushing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-seven adult orthodontic patients with fixed orthodontic appliances were divided into three study groups : ( 1 ) oral irrigation with automatic toothbrush , ( n = 16 ) ; ( 2 ) oral irrigation with manual toothbrushing , ( n = 16 ) ; ( 3 ) control group with continued normal toothbrushing only , ( n = 15 ) .
	manualset3
230738	14	428033	15	NULL	NULL	0	NULL	n = 15	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-seven adult orthodontic patients with fixed orthodontic appliances were divided into three study groups : ( 1 ) oral irrigation with automatic toothbrush , ( n = 16 ) ; ( 2 ) oral irrigation with manual toothbrushing , ( n = 16 ) ; ( 3 ) control group with continued normal toothbrushing only , ( n = 15 ) .
	manualset3
230739	1	428034	15	NULL	NULL	0	NULL	Forty-three adult cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-three adult cases of acute leukemia ( AL ) seen at the University of Benin Teaching Hospital , Benin City , Nigeria in the 13-year period 1975-1987 have been analyzed with respect to the presenting features , management and outcome .
	manualset3
230740	2	428034	15	NULL	NULL	0	NULL	acute leukemia ( AL ) 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-three adult cases of acute leukemia ( AL ) seen at the University of Benin Teaching Hospital , Benin City , Nigeria in the 13-year period 1975-1987 have been analyzed with respect to the presenting features , management and outcome .
	manualset3
230741	3	428034	15	NULL	NULL	0	NULL	University of Benin Teaching Hospital	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-three adult cases of acute leukemia ( AL ) seen at the University of Benin Teaching Hospital , Benin City , Nigeria in the 13-year period 1975-1987 have been analyzed with respect to the presenting features , management and outcome .
	manualset3
230743	5	428034	15	NULL	NULL	0	NULL	Benin City , Nigeria	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-three adult cases of acute leukemia ( AL ) seen at the University of Benin Teaching Hospital , Benin City , Nigeria in the 13-year period 1975-1987 have been analyzed with respect to the presenting features , management and outcome .
	manualset3
230744	6	428034	15	NULL	NULL	0	NULL	13-year period	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-three adult cases of acute leukemia ( AL ) seen at the University of Benin Teaching Hospital , Benin City , Nigeria in the 13-year period 1975-1987 have been analyzed with respect to the presenting features , management and outcome .
	manualset3
230745	7	428034	15	NULL	NULL	0	NULL	1975-1987	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-three adult cases of acute leukemia ( AL ) seen at the University of Benin Teaching Hospital , Benin City , Nigeria in the 13-year period 1975-1987 have been analyzed with respect to the presenting features , management and outcome .
	manualset3
230746	8	428034	15	NULL	NULL	NULL	NULL	presenting features	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Forty-three adult cases of acute leukemia ( AL ) seen at the University of Benin Teaching Hospital , Benin City , Nigeria in the 13-year period 1975-1987 have been analyzed with respect to the presenting features , management and outcome .
	manualset3
230747	9	428034	15	NULL	NULL	NULL	NULL	management	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Forty-three adult cases of acute leukemia ( AL ) seen at the University of Benin Teaching Hospital , Benin City , Nigeria in the 13-year period 1975-1987 have been analyzed with respect to the presenting features , management and outcome .
	manualset3
230748	10	428034	15	NULL	NULL	NULL	NULL	outcome	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Forty-three adult cases of acute leukemia ( AL ) seen at the University of Benin Teaching Hospital , Benin City , Nigeria in the 13-year period 1975-1987 have been analyzed with respect to the presenting features , management and outcome .
	manualset3
230749	1	428035	15	NULL	NULL	0	NULL	Research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Research on the relevance of earthworms inducing soil Cd2 + absorbed by perennial ryegrass ) .
	manualset3
230750	2	428035	15	NULL	NULL	0	NULL	relevance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Research on the relevance of earthworms inducing soil Cd2 + absorbed by perennial ryegrass ) .
	manualset3
230751	3	428035	15	NULL	NULL	0	NULL	earthworms	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Research on the relevance of earthworms inducing soil Cd2 + absorbed by perennial ryegrass ) .
	manualset3
230753	4	428035	15	NULL	NULL	0	NULL	soil 	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	( Research on the relevance of earthworms inducing soil Cd2 + absorbed by perennial ryegrass ) .
	manualset3
230754	5	428035	15	NULL	NULL	0	NULL	Cd2 +	Ion												NULL		0	NULL	NULL	NULL	NULL	NULL	( Research on the relevance of earthworms inducing soil Cd2 + absorbed by perennial ryegrass ) .
	manualset3
230755	6	428035	15	NULL	NULL	NULL	NULL	perennial ryegrass	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Research on the relevance of earthworms inducing soil Cd2 + absorbed by perennial ryegrass ) .
	manualset3
230358	1	428036	15	NULL	NULL	NULL	NULL	Forty-two patients 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Forty-two patients ( 72.4 % ) had a complete response to therapy .
	manualset3
230483	2	428036	15	NULL	NULL	0	NULL	72.4 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-two patients ( 72.4 % ) had a complete response to therapy .
	manualset3
230484	3	428036	15	NULL	NULL	0	NULL	response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-two patients ( 72.4 % ) had a complete response to therapy .
	manualset3
230485	4	428036	15	NULL	NULL	0	NULL	therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Forty-two patients ( 72.4 % ) had a complete response to therapy .
	manualset3
230361	1	428037	15	NULL	NULL	0	NULL	Fos	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Fos expression was significantly different between intact and zinc sulfate-treated anosmic mating males in only one area studied .
	manualset3
230362	2	428037	15	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fos expression was significantly different between intact and zinc sulfate-treated anosmic mating males in only one area studied .
	manualset3
230363	3	428037	15	NULL	NULL	0	NULL	zinc sulfate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Fos expression was significantly different between intact and zinc sulfate-treated anosmic mating males in only one area studied .
	manualset3
230366	6	428037	15	NULL	NULL	0	NULL	area	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Fos expression was significantly different between intact and zinc sulfate-treated anosmic mating males in only one area studied .
	manualset3
230486	4	428037	15	NULL	NULL	0	NULL	anosmic mating males	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Fos expression was significantly different between intact and zinc sulfate-treated anosmic mating males in only one area studied .
	manualset3
230487	5	428037	15	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Fos expression was significantly different between intact and zinc sulfate-treated anosmic mating males in only one area studied .
	manualset3
230367	1	428038	15	NULL	NULL	NULL	NULL	Four	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four-wave mixing with large stokes shifts in heavily Ge-doped silica fibers .
	manualset3
230488	2	428038	15	NULL	NULL	0	NULL	wave mixing	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Four-wave mixing with large stokes shifts in heavily Ge-doped silica fibers .
	manualset3
230489	3	428038	15	NULL	NULL	0	NULL	shifts	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Four-wave mixing with large stokes shifts in heavily Ge-doped silica fibers .
	manualset3
230490	4	428038	15	NULL	NULL	0	NULL	Ge-doped silica fibers	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Four-wave mixing with large stokes shifts in heavily Ge-doped silica fibers .
	manualset3
230379	1	428039	15	NULL	NULL	NULL	NULL	Four-week-old male Wistar rats	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four-week-old male Wistar rats received a single subcutaneous injection of 60 mg/kg monocrotaline and were then chronically and subcutaneously infused with rat adrenomedullin ( PH + AM group , n = 8 ) or saline ( PH group , n = 10 ) by an osmotic minipump for a period of 21 days .
	manualset3
230380	3	428039	15	NULL	NULL	NULL	NULL	60 mg/kg	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four-week-old male Wistar rats received a single subcutaneous injection of 60 mg/kg monocrotaline and were then chronically and subcutaneously infused with rat adrenomedullin ( PH + AM group , n = 8 ) or saline ( PH group , n = 10 ) by an osmotic minipump for a period of 21 days .
	manualset3
230381	4	428039	15	NULL	NULL	NULL	NULL	monocrotaline	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four-week-old male Wistar rats received a single subcutaneous injection of 60 mg/kg monocrotaline and were then chronically and subcutaneously infused with rat adrenomedullin ( PH + AM group , n = 8 ) or saline ( PH group , n = 10 ) by an osmotic minipump for a period of 21 days .
	manualset3
230384	5	428039	15	NULL	NULL	NULL	NULL	rat 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four-week-old male Wistar rats received a single subcutaneous injection of 60 mg/kg monocrotaline and were then chronically and subcutaneously infused with rat adrenomedullin ( PH + AM group , n = 8 ) or saline ( PH group , n = 10 ) by an osmotic minipump for a period of 21 days .
	manualset3
230390	6	428039	15	NULL	NULL	NULL	NULL	adrenomedullin	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four-week-old male Wistar rats received a single subcutaneous injection of 60 mg/kg monocrotaline and were then chronically and subcutaneously infused with rat adrenomedullin ( PH + AM group , n = 8 ) or saline ( PH group , n = 10 ) by an osmotic minipump for a period of 21 days .
	manualset3
230491	2	428039	15	NULL	NULL	0	NULL	single subcutaneous injection 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Four-week-old male Wistar rats received a single subcutaneous injection of 60 mg/kg monocrotaline and were then chronically and subcutaneously infused with rat adrenomedullin ( PH + AM group , n = 8 ) or saline ( PH group , n = 10 ) by an osmotic minipump for a period of 21 days .
	manualset3
230492	7	428039	15	NULL	NULL	0	NULL	PH + AM group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Four-week-old male Wistar rats received a single subcutaneous injection of 60 mg/kg monocrotaline and were then chronically and subcutaneously infused with rat adrenomedullin ( PH + AM group , n = 8 ) or saline ( PH group , n = 10 ) by an osmotic minipump for a period of 21 days .
	manualset3
230494	8	428039	15	NULL	NULL	0	NULL	n = 8	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Four-week-old male Wistar rats received a single subcutaneous injection of 60 mg/kg monocrotaline and were then chronically and subcutaneously infused with rat adrenomedullin ( PH + AM group , n = 8 ) or saline ( PH group , n = 10 ) by an osmotic minipump for a period of 21 days .
	manualset3
230495	9	428039	15	NULL	NULL	0	NULL	saline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Four-week-old male Wistar rats received a single subcutaneous injection of 60 mg/kg monocrotaline and were then chronically and subcutaneously infused with rat adrenomedullin ( PH + AM group , n = 8 ) or saline ( PH group , n = 10 ) by an osmotic minipump for a period of 21 days .
	manualset3
230496	10	428039	15	NULL	NULL	0	NULL	 PH group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Four-week-old male Wistar rats received a single subcutaneous injection of 60 mg/kg monocrotaline and were then chronically and subcutaneously infused with rat adrenomedullin ( PH + AM group , n = 8 ) or saline ( PH group , n = 10 ) by an osmotic minipump for a period of 21 days .
	manualset3
230497	11	428039	15	NULL	NULL	0	NULL	n = 10 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Four-week-old male Wistar rats received a single subcutaneous injection of 60 mg/kg monocrotaline and were then chronically and subcutaneously infused with rat adrenomedullin ( PH + AM group , n = 8 ) or saline ( PH group , n = 10 ) by an osmotic minipump for a period of 21 days .
	manualset3
230498	12	428039	15	NULL	NULL	0	NULL	osmotic minipump	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	Four-week-old male Wistar rats received a single subcutaneous injection of 60 mg/kg monocrotaline and were then chronically and subcutaneously infused with rat adrenomedullin ( PH + AM group , n = 8 ) or saline ( PH group , n = 10 ) by an osmotic minipump for a period of 21 days .
	manualset3
230499	13	428039	15	NULL	NULL	0	NULL	period 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Four-week-old male Wistar rats received a single subcutaneous injection of 60 mg/kg monocrotaline and were then chronically and subcutaneously infused with rat adrenomedullin ( PH + AM group , n = 8 ) or saline ( PH group , n = 10 ) by an osmotic minipump for a period of 21 days .
	manualset3
230500	14	428039	15	NULL	NULL	0	NULL	21 days	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Four-week-old male Wistar rats received a single subcutaneous injection of 60 mg/kg monocrotaline and were then chronically and subcutaneously infused with rat adrenomedullin ( PH + AM group , n = 8 ) or saline ( PH group , n = 10 ) by an osmotic minipump for a period of 21 days .
	manualset3
230417	1	428040	15	NULL	NULL	0	NULL	Research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Research on the suitability of peptones for testing of hydrogen sulfide formation by Brucellae ) .
	manualset3
230425	3	428040	15	NULL	NULL	NULL	NULL	peptones	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Research on the suitability of peptones for testing of hydrogen sulfide formation by Brucellae ) .
	manualset3
230426	5	428040	15	NULL	NULL	NULL	NULL	hydrogen sulfide	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Research on the suitability of peptones for testing of hydrogen sulfide formation by Brucellae ) .
	manualset3
230427	7	428040	15	NULL	NULL	NULL	NULL	Brucellae	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Research on the suitability of peptones for testing of hydrogen sulfide formation by Brucellae ) .
	manualset3
230501	2	428040	15	NULL	NULL	NULL	NULL	suitability	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Research on the suitability of peptones for testing of hydrogen sulfide formation by Brucellae ) .
	manualset3
230502	4	428040	15	NULL	NULL	0	NULL	testing	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Research on the suitability of peptones for testing of hydrogen sulfide formation by Brucellae ) .
	manualset3
230503	6	428040	15	NULL	NULL	0	NULL	formation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Research on the suitability of peptones for testing of hydrogen sulfide formation by Brucellae ) .
	manualset3
230504	1	428041	15	NULL	NULL	0	NULL	Four-week treatment response	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Four-week treatment response of all patients was compared with pretreatment HPA axis variables , and higher cortisol values after dexamethasone administration were found to be significantly correlated with greater improvement .
	manualset3
230505	2	428041	15	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Four-week treatment response of all patients was compared with pretreatment HPA axis variables , and higher cortisol values after dexamethasone administration were found to be significantly correlated with greater improvement .
	manualset3
230506	3	428041	15	NULL	NULL	0	NULL	pretreatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Four-week treatment response of all patients was compared with pretreatment HPA axis variables , and higher cortisol values after dexamethasone administration were found to be significantly correlated with greater improvement .
	manualset3
230507	4	428041	15	NULL	NULL	0	NULL	HPA axis variables	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Four-week treatment response of all patients was compared with pretreatment HPA axis variables , and higher cortisol values after dexamethasone administration were found to be significantly correlated with greater improvement .
	manualset3
230508	5	428041	15	NULL	NULL	0	NULL	higher cortisol values	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Four-week treatment response of all patients was compared with pretreatment HPA axis variables , and higher cortisol values after dexamethasone administration were found to be significantly correlated with greater improvement .
	manualset3
230509	6	428041	15	NULL	NULL	0	NULL	dexamethasone	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Four-week treatment response of all patients was compared with pretreatment HPA axis variables , and higher cortisol values after dexamethasone administration were found to be significantly correlated with greater improvement .
	manualset3
230510	7	428041	15	NULL	NULL	0	NULL	administration	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Four-week treatment response of all patients was compared with pretreatment HPA axis variables , and higher cortisol values after dexamethasone administration were found to be significantly correlated with greater improvement .
	manualset3
230511	8	428041	15	NULL	NULL	NULL	NULL	improvement 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four-week treatment response of all patients was compared with pretreatment HPA axis variables , and higher cortisol values after dexamethasone administration were found to be significantly correlated with greater improvement .
	manualset3
230513	1	428042	15	NULL	NULL	NULL	NULL	Four C residues	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four C residues are edited into U , resulting in the creation of a putative translational initiation codon , a new stop codon which eliminated ten carboxy-terminal residues , and two additional amino-acid alterations .
	manualset3
230515	2	428042	15	NULL	NULL	NULL	NULL	U	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four C residues are edited into U , resulting in the creation of a putative translational initiation codon , a new stop codon which eliminated ten carboxy-terminal residues , and two additional amino-acid alterations .
	manualset3
230516	3	428042	15	NULL	NULL	NULL	NULL	creation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four C residues are edited into U , resulting in the creation of a putative translational initiation codon , a new stop codon which eliminated ten carboxy-terminal residues , and two additional amino-acid alterations .
	manualset3
230517	4	428042	15	NULL	NULL	NULL	NULL	putative translational initiation codon	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four C residues are edited into U , resulting in the creation of a putative translational initiation codon , a new stop codon which eliminated ten carboxy-terminal residues , and two additional amino-acid alterations .
	manualset3
230518	5	428042	15	NULL	NULL	NULL	NULL	stop codon	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four C residues are edited into U , resulting in the creation of a putative translational initiation codon , a new stop codon which eliminated ten carboxy-terminal residues , and two additional amino-acid alterations .
	manualset3
230520	6	428042	15	NULL	NULL	NULL	NULL	ten carboxy-terminal residues 	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four C residues are edited into U , resulting in the creation of a putative translational initiation codon , a new stop codon which eliminated ten carboxy-terminal residues , and two additional amino-acid alterations .
	manualset3
230521	7	428042	15	NULL	NULL	NULL	NULL	two	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four C residues are edited into U , resulting in the creation of a putative translational initiation codon , a new stop codon which eliminated ten carboxy-terminal residues , and two additional amino-acid alterations .
	manualset3
230523	8	428042	15	NULL	NULL	NULL	NULL	amino-acid alterations	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four C residues are edited into U , resulting in the creation of a putative translational initiation codon , a new stop codon which eliminated ten carboxy-terminal residues , and two additional amino-acid alterations .
	manualset3
230524	1	428043	15	NULL	NULL	0	NULL	Four	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four Syke 's monkeys ( Cercopithecus mitis ) , two vervet monkeys ( Cercopithecus aethiops ) , two baboons ( Papio cynocephalus ) , and two brown bushbabies ( Galago garnettii ) were each inoculated intradermally on the left eyelid , left ear , and nose with 0.1 ml of medium containing 1 x 10 ( 7 ) promastigotes of a characterized L. major strain .
	manualset3
230525	2	428043	15	NULL	NULL	0	NULL	Syke 's monkeys	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Four Syke 's monkeys ( Cercopithecus mitis ) , two vervet monkeys ( Cercopithecus aethiops ) , two baboons ( Papio cynocephalus ) , and two brown bushbabies ( Galago garnettii ) were each inoculated intradermally on the left eyelid , left ear , and nose with 0.1 ml of medium containing 1 x 10 ( 7 ) promastigotes of a characterized L. major strain .
	manualset3
230527	3	428043	15	NULL	NULL	0	NULL	Cercopithecus mitis	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Four Syke 's monkeys ( Cercopithecus mitis ) , two vervet monkeys ( Cercopithecus aethiops ) , two baboons ( Papio cynocephalus ) , and two brown bushbabies ( Galago garnettii ) were each inoculated intradermally on the left eyelid , left ear , and nose with 0.1 ml of medium containing 1 x 10 ( 7 ) promastigotes of a characterized L. major strain .
	manualset3
230528	4	428043	15	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four Syke 's monkeys ( Cercopithecus mitis ) , two vervet monkeys ( Cercopithecus aethiops ) , two baboons ( Papio cynocephalus ) , and two brown bushbabies ( Galago garnettii ) were each inoculated intradermally on the left eyelid , left ear , and nose with 0.1 ml of medium containing 1 x 10 ( 7 ) promastigotes of a characterized L. major strain .
	manualset3
230529	5	428043	15	NULL	NULL	0	NULL	vervet monkeys	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Four Syke 's monkeys ( Cercopithecus mitis ) , two vervet monkeys ( Cercopithecus aethiops ) , two baboons ( Papio cynocephalus ) , and two brown bushbabies ( Galago garnettii ) were each inoculated intradermally on the left eyelid , left ear , and nose with 0.1 ml of medium containing 1 x 10 ( 7 ) promastigotes of a characterized L. major strain .
	manualset3
230530	6	428043	15	NULL	NULL	0	NULL	Cercopithecus aethiops	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Four Syke 's monkeys ( Cercopithecus mitis ) , two vervet monkeys ( Cercopithecus aethiops ) , two baboons ( Papio cynocephalus ) , and two brown bushbabies ( Galago garnettii ) were each inoculated intradermally on the left eyelid , left ear , and nose with 0.1 ml of medium containing 1 x 10 ( 7 ) promastigotes of a characterized L. major strain .
	manualset3
230531	7	428043	15	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four Syke 's monkeys ( Cercopithecus mitis ) , two vervet monkeys ( Cercopithecus aethiops ) , two baboons ( Papio cynocephalus ) , and two brown bushbabies ( Galago garnettii ) were each inoculated intradermally on the left eyelid , left ear , and nose with 0.1 ml of medium containing 1 x 10 ( 7 ) promastigotes of a characterized L. major strain .
	manualset3
230532	8	428043	15	NULL	NULL	0	NULL	baboons	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Four Syke 's monkeys ( Cercopithecus mitis ) , two vervet monkeys ( Cercopithecus aethiops ) , two baboons ( Papio cynocephalus ) , and two brown bushbabies ( Galago garnettii ) were each inoculated intradermally on the left eyelid , left ear , and nose with 0.1 ml of medium containing 1 x 10 ( 7 ) promastigotes of a characterized L. major strain .
	manualset3
230533	9	428043	15	NULL	NULL	0	NULL	Papio cynocephalus	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Four Syke 's monkeys ( Cercopithecus mitis ) , two vervet monkeys ( Cercopithecus aethiops ) , two baboons ( Papio cynocephalus ) , and two brown bushbabies ( Galago garnettii ) were each inoculated intradermally on the left eyelid , left ear , and nose with 0.1 ml of medium containing 1 x 10 ( 7 ) promastigotes of a characterized L. major strain .
	manualset3
230534	10	428043	15	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four Syke 's monkeys ( Cercopithecus mitis ) , two vervet monkeys ( Cercopithecus aethiops ) , two baboons ( Papio cynocephalus ) , and two brown bushbabies ( Galago garnettii ) were each inoculated intradermally on the left eyelid , left ear , and nose with 0.1 ml of medium containing 1 x 10 ( 7 ) promastigotes of a characterized L. major strain .
	manualset3
230535	11	428043	15	NULL	NULL	0	NULL	brown bushbabies	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Four Syke 's monkeys ( Cercopithecus mitis ) , two vervet monkeys ( Cercopithecus aethiops ) , two baboons ( Papio cynocephalus ) , and two brown bushbabies ( Galago garnettii ) were each inoculated intradermally on the left eyelid , left ear , and nose with 0.1 ml of medium containing 1 x 10 ( 7 ) promastigotes of a characterized L. major strain .
	manualset3
230537	12	428043	15	NULL	NULL	0	NULL	Galago garnettii	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Four Syke 's monkeys ( Cercopithecus mitis ) , two vervet monkeys ( Cercopithecus aethiops ) , two baboons ( Papio cynocephalus ) , and two brown bushbabies ( Galago garnettii ) were each inoculated intradermally on the left eyelid , left ear , and nose with 0.1 ml of medium containing 1 x 10 ( 7 ) promastigotes of a characterized L. major strain .
	manualset3
230538	13	428043	15	NULL	NULL	0	NULL	left eyelid	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Four Syke 's monkeys ( Cercopithecus mitis ) , two vervet monkeys ( Cercopithecus aethiops ) , two baboons ( Papio cynocephalus ) , and two brown bushbabies ( Galago garnettii ) were each inoculated intradermally on the left eyelid , left ear , and nose with 0.1 ml of medium containing 1 x 10 ( 7 ) promastigotes of a characterized L. major strain .
	manualset3
230539	14	428043	15	NULL	NULL	0	NULL	left ear	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Four Syke 's monkeys ( Cercopithecus mitis ) , two vervet monkeys ( Cercopithecus aethiops ) , two baboons ( Papio cynocephalus ) , and two brown bushbabies ( Galago garnettii ) were each inoculated intradermally on the left eyelid , left ear , and nose with 0.1 ml of medium containing 1 x 10 ( 7 ) promastigotes of a characterized L. major strain .
	manualset3
230541	15	428043	15	NULL	NULL	0	NULL	nose	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Four Syke 's monkeys ( Cercopithecus mitis ) , two vervet monkeys ( Cercopithecus aethiops ) , two baboons ( Papio cynocephalus ) , and two brown bushbabies ( Galago garnettii ) were each inoculated intradermally on the left eyelid , left ear , and nose with 0.1 ml of medium containing 1 x 10 ( 7 ) promastigotes of a characterized L. major strain .
	manualset3
230542	16	428043	15	NULL	NULL	0	NULL	0.1 ml 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Four Syke 's monkeys ( Cercopithecus mitis ) , two vervet monkeys ( Cercopithecus aethiops ) , two baboons ( Papio cynocephalus ) , and two brown bushbabies ( Galago garnettii ) were each inoculated intradermally on the left eyelid , left ear , and nose with 0.1 ml of medium containing 1 x 10 ( 7 ) promastigotes of a characterized L. major strain .
	manualset3
230545	17	428043	15	NULL	NULL	0	NULL	medium	LaboratoryExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Four Syke 's monkeys ( Cercopithecus mitis ) , two vervet monkeys ( Cercopithecus aethiops ) , two baboons ( Papio cynocephalus ) , and two brown bushbabies ( Galago garnettii ) were each inoculated intradermally on the left eyelid , left ear , and nose with 0.1 ml of medium containing 1 x 10 ( 7 ) promastigotes of a characterized L. major strain .
	manualset3
230547	18	428043	15	NULL	NULL	0	NULL	1 x 10 ( 7 )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four Syke 's monkeys ( Cercopithecus mitis ) , two vervet monkeys ( Cercopithecus aethiops ) , two baboons ( Papio cynocephalus ) , and two brown bushbabies ( Galago garnettii ) were each inoculated intradermally on the left eyelid , left ear , and nose with 0.1 ml of medium containing 1 x 10 ( 7 ) promastigotes of a characterized L. major strain .
	manualset3
230550	19	428043	15	NULL	NULL	NULL	NULL	promastigotes	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four Syke 's monkeys ( Cercopithecus mitis ) , two vervet monkeys ( Cercopithecus aethiops ) , two baboons ( Papio cynocephalus ) , and two brown bushbabies ( Galago garnettii ) were each inoculated intradermally on the left eyelid , left ear , and nose with 0.1 ml of medium containing 1 x 10 ( 7 ) promastigotes of a characterized L. major strain .
	manualset3
230551	20	428043	15	NULL	NULL	0	NULL	L. major strain	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Four Syke 's monkeys ( Cercopithecus mitis ) , two vervet monkeys ( Cercopithecus aethiops ) , two baboons ( Papio cynocephalus ) , and two brown bushbabies ( Galago garnettii ) were each inoculated intradermally on the left eyelid , left ear , and nose with 0.1 ml of medium containing 1 x 10 ( 7 ) promastigotes of a characterized L. major strain .
	manualset3
230553	1	428044	15	NULL	NULL	0	NULL	Four	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four alpha-dicarbonyl compounds , aldehydic and ketonic , were reacted with the modified amino acid N ( alpha ) - acetyl-L-arginine ( AcArg ) , in an attempt to establish structure/activity relationships for the reactivity of alpha-dicarbonyls with the amine compound .
	manualset3
230555	2	428044	15	NULL	NULL	0	NULL	alpha-dicarbonyl compounds	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Four alpha-dicarbonyl compounds , aldehydic and ketonic , were reacted with the modified amino acid N ( alpha ) - acetyl-L-arginine ( AcArg ) , in an attempt to establish structure/activity relationships for the reactivity of alpha-dicarbonyls with the amine compound .
	manualset3
230557	3	428044	15	NULL	NULL	0	NULL	amino acid N ( alpha ) - acetyl-L-arginine ( AcArg )	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Four alpha-dicarbonyl compounds , aldehydic and ketonic , were reacted with the modified amino acid N ( alpha ) - acetyl-L-arginine ( AcArg ) , in an attempt to establish structure/activity relationships for the reactivity of alpha-dicarbonyls with the amine compound .
	manualset3
230559	5	428044	15	NULL	NULL	NULL	NULL	structure/activity relationships	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four alpha-dicarbonyl compounds , aldehydic and ketonic , were reacted with the modified amino acid N ( alpha ) - acetyl-L-arginine ( AcArg ) , in an attempt to establish structure/activity relationships for the reactivity of alpha-dicarbonyls with the amine compound .
	manualset3
230560	6	428044	15	NULL	NULL	NULL	NULL	reactivity	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four alpha-dicarbonyl compounds , aldehydic and ketonic , were reacted with the modified amino acid N ( alpha ) - acetyl-L-arginine ( AcArg ) , in an attempt to establish structure/activity relationships for the reactivity of alpha-dicarbonyls with the amine compound .
	manualset3
230561	7	428044	15	NULL	NULL	NULL	NULL	alpha-dicarbonyls 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four alpha-dicarbonyl compounds , aldehydic and ketonic , were reacted with the modified amino acid N ( alpha ) - acetyl-L-arginine ( AcArg ) , in an attempt to establish structure/activity relationships for the reactivity of alpha-dicarbonyls with the amine compound .
	manualset3
230562	8	428044	15	NULL	NULL	NULL	NULL	amine compound	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four alpha-dicarbonyl compounds , aldehydic and ketonic , were reacted with the modified amino acid N ( alpha ) - acetyl-L-arginine ( AcArg ) , in an attempt to establish structure/activity relationships for the reactivity of alpha-dicarbonyls with the amine compound .
	manualset3
234400	4	428044	15	NULL	NULL	0	NULL	attempt 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Four alpha-dicarbonyl compounds , aldehydic and ketonic , were reacted with the modified amino acid N ( alpha ) - acetyl-L-arginine ( AcArg ) , in an attempt to establish structure/activity relationships for the reactivity of alpha-dicarbonyls with the amine compound .
	manualset3
230678	1	428045	15	NULL	NULL	0	NULL	Four cases	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four cases are discussed , with the point in view that examination of oral cavity , trachea , hands and all injuries is a vital part of post-mortem examination for the administration of justice .
	manualset3
230679	3	428045	15	NULL	NULL	NULL	NULL	examination	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four cases are discussed , with the point in view that examination of oral cavity , trachea , hands and all injuries is a vital part of post-mortem examination for the administration of justice .
	manualset3
230680	4	428045	15	NULL	NULL	NULL	NULL	oral cavity	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four cases are discussed , with the point in view that examination of oral cavity , trachea , hands and all injuries is a vital part of post-mortem examination for the administration of justice .
	manualset3
230681	5	428045	15	NULL	NULL	NULL	NULL	trachea	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four cases are discussed , with the point in view that examination of oral cavity , trachea , hands and all injuries is a vital part of post-mortem examination for the administration of justice .
	manualset3
230682	6	428045	15	NULL	NULL	NULL	NULL	hands	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four cases are discussed , with the point in view that examination of oral cavity , trachea , hands and all injuries is a vital part of post-mortem examination for the administration of justice .
	manualset3
230683	7	428045	15	NULL	NULL	NULL	NULL	injuries	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four cases are discussed , with the point in view that examination of oral cavity , trachea , hands and all injuries is a vital part of post-mortem examination for the administration of justice .
	manualset3
230684	9	428045	15	NULL	NULL	NULL	NULL	post-mortem examination	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four cases are discussed , with the point in view that examination of oral cavity , trachea , hands and all injuries is a vital part of post-mortem examination for the administration of justice .
	manualset3
230685	10	428045	15	NULL	NULL	NULL	NULL	administration	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four cases are discussed , with the point in view that examination of oral cavity , trachea , hands and all injuries is a vital part of post-mortem examination for the administration of justice .
	manualset3
230812	2	428045	15	NULL	NULL	NULL	NULL	view	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four cases are discussed , with the point in view that examination of oral cavity , trachea , hands and all injuries is a vital part of post-mortem examination for the administration of justice .
	manualset3
230828	8	428045	15	NULL	NULL	0	NULL	vital part	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Four cases are discussed , with the point in view that examination of oral cavity , trachea , hands and all injuries is a vital part of post-mortem examination for the administration of justice .
	manualset3
230833	11	428045	15	NULL	NULL	0	NULL	justice	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Four cases are discussed , with the point in view that examination of oral cavity , trachea , hands and all injuries is a vital part of post-mortem examination for the administration of justice .
	manualset3
230686	1	428046	15	NULL	NULL	0	NULL	Four cases	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four cases died , two cases of pulmonary tuberculosis died from hemoptysis , and two cases of atypical mycobacteriosis died from respiratory failure .
	manualset3
230687	2	428046	15	NULL	NULL	0	NULL	two cases	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four cases died , two cases of pulmonary tuberculosis died from hemoptysis , and two cases of atypical mycobacteriosis died from respiratory failure .
	manualset3
230688	3	428046	15	NULL	NULL	0	NULL	pulmonary tuberculosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Four cases died , two cases of pulmonary tuberculosis died from hemoptysis , and two cases of atypical mycobacteriosis died from respiratory failure .
	manualset3
230689	4	428046	15	NULL	NULL	0	NULL	hemoptysis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Four cases died , two cases of pulmonary tuberculosis died from hemoptysis , and two cases of atypical mycobacteriosis died from respiratory failure .
	manualset3
230690	5	428046	15	NULL	NULL	0	NULL	two cases	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four cases died , two cases of pulmonary tuberculosis died from hemoptysis , and two cases of atypical mycobacteriosis died from respiratory failure .
	manualset3
230691	6	428046	15	NULL	NULL	0	NULL	atypical mycobacteriosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Four cases died , two cases of pulmonary tuberculosis died from hemoptysis , and two cases of atypical mycobacteriosis died from respiratory failure .
	manualset3
230692	7	428046	15	NULL	NULL	0	NULL	respiratory failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Four cases died , two cases of pulmonary tuberculosis died from hemoptysis , and two cases of atypical mycobacteriosis died from respiratory failure .
	manualset3
230693	1	428047	15	NULL	NULL	0	NULL	Four cases	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four cases died of regional failure without any metastatic lesions ( survival ranged from 5 months to 22 months ) .
	manualset3
230694	2	428047	15	NULL	NULL	0	NULL	regional failure	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Four cases died of regional failure without any metastatic lesions ( survival ranged from 5 months to 22 months ) .
	manualset3
230695	3	428047	15	NULL	NULL	0	NULL	metastatic lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Four cases died of regional failure without any metastatic lesions ( survival ranged from 5 months to 22 months ) .
	manualset3
230696	4	428047	15	NULL	NULL	0	NULL	survival	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Four cases died of regional failure without any metastatic lesions ( survival ranged from 5 months to 22 months ) .
	manualset3
230697	5	428047	15	NULL	NULL	0	NULL	5 months to 22 months 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Four cases died of regional failure without any metastatic lesions ( survival ranged from 5 months to 22 months ) .
	manualset3
230698	1	428048	15	NULL	NULL	0	NULL	Four cases	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four cases encountered in routine autopsy evaluation at our institute in 2004 in which non-atherosclerotic coronary pathology was responsible for sudden cardiac death are reported .
	manualset3
230699	2	428048	15	NULL	NULL	0	NULL	autopsy evaluation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Four cases encountered in routine autopsy evaluation at our institute in 2004 in which non-atherosclerotic coronary pathology was responsible for sudden cardiac death are reported .
	manualset3
230700	3	428048	15	NULL	NULL	0	NULL	institute	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Four cases encountered in routine autopsy evaluation at our institute in 2004 in which non-atherosclerotic coronary pathology was responsible for sudden cardiac death are reported .
	manualset3
230701	4	428048	15	NULL	NULL	0	NULL	2004	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	Four cases encountered in routine autopsy evaluation at our institute in 2004 in which non-atherosclerotic coronary pathology was responsible for sudden cardiac death are reported .
	manualset3
230702	5	428048	15	NULL	NULL	0	NULL	non-atherosclerotic coronary pathology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Four cases encountered in routine autopsy evaluation at our institute in 2004 in which non-atherosclerotic coronary pathology was responsible for sudden cardiac death are reported .
	manualset3
230703	6	428048	15	NULL	NULL	NULL	NULL	sudden cardiac death	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four cases encountered in routine autopsy evaluation at our institute in 2004 in which non-atherosclerotic coronary pathology was responsible for sudden cardiac death are reported .
	manualset3
230704	1	428049	15	NULL	NULL	0	NULL	Four cases	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four cases had deletions that ended proximal to HMGA2 and all of these had much better growth .
	manualset3
230705	2	428049	15	NULL	NULL	0	NULL	deletions	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Four cases had deletions that ended proximal to HMGA2 and all of these had much better growth .
	manualset3
230706	3	428049	15	NULL	NULL	0	NULL	HMGA2	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Four cases had deletions that ended proximal to HMGA2 and all of these had much better growth .
	manualset3
230708	4	428049	15	NULL	NULL	NULL	NULL	growth	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four cases had deletions that ended proximal to HMGA2 and all of these had much better growth .
	manualset3
230709	1	428050	15	NULL	NULL	0	NULL	Four cases	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four cases were embolized and one very small extradural aneurysm is still not treated .
	manualset3
230710	2	428050	15	NULL	NULL	0	NULL	one 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four cases were embolized and one very small extradural aneurysm is still not treated .
	manualset3
230711	3	428050	15	NULL	NULL	0	NULL	extradural aneurysm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Four cases were embolized and one very small extradural aneurysm is still not treated .
	manualset3
230821	1	428051	15	NULL	NULL	0	NULL	Research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Research on correlations between immuno-nutritional parameters and oncologic stage in patients operated on for cancer of the stomach ) .
	manualset3
230822	2	428051	15	NULL	NULL	0	NULL	correlations	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	( Research on correlations between immuno-nutritional parameters and oncologic stage in patients operated on for cancer of the stomach ) .
	manualset3
230836	3	428051	15	NULL	NULL	NULL	NULL	immuno-nutritional parameters	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Research on correlations between immuno-nutritional parameters and oncologic stage in patients operated on for cancer of the stomach ) .
	manualset3
230838	4	428051	15	NULL	NULL	0	NULL	oncologic stage	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Research on correlations between immuno-nutritional parameters and oncologic stage in patients operated on for cancer of the stomach ) .
	manualset3
230840	5	428051	15	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Research on correlations between immuno-nutritional parameters and oncologic stage in patients operated on for cancer of the stomach ) .
	manualset3
230843	6	428051	15	NULL	NULL	0	NULL	cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Research on correlations between immuno-nutritional parameters and oncologic stage in patients operated on for cancer of the stomach ) .
	manualset3
230844	7	428051	15	NULL	NULL	0	NULL	stomach	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Research on correlations between immuno-nutritional parameters and oncologic stage in patients operated on for cancer of the stomach ) .
	manualset3
230849	1	428052	15	NULL	NULL	0	NULL	Four coastal Aboriginal settlements	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four coastal Aboriginal settlements in the northwest area of Australia have been investigated for plasma trace metal status -- Zinc ( Zn ) , Copper ( Cu ) , and Iron ( Fe ) .
	manualset3
230853	2	428052	15	NULL	NULL	0	NULL	northwest area of Australia	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Four coastal Aboriginal settlements in the northwest area of Australia have been investigated for plasma trace metal status -- Zinc ( Zn ) , Copper ( Cu ) , and Iron ( Fe ) .
	manualset3
230857	3	428052	15	NULL	NULL	0	NULL	plasma trace metal status	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Four coastal Aboriginal settlements in the northwest area of Australia have been investigated for plasma trace metal status -- Zinc ( Zn ) , Copper ( Cu ) , and Iron ( Fe ) .
	manualset3
230862	4	428052	15	NULL	NULL	0	NULL	Zinc ( Zn )	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Four coastal Aboriginal settlements in the northwest area of Australia have been investigated for plasma trace metal status -- Zinc ( Zn ) , Copper ( Cu ) , and Iron ( Fe ) .
	manualset3
230863	5	428052	15	NULL	NULL	0	NULL	Copper ( Cu )	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Four coastal Aboriginal settlements in the northwest area of Australia have been investigated for plasma trace metal status -- Zinc ( Zn ) , Copper ( Cu ) , and Iron ( Fe ) .
	manualset3
230864	6	428052	15	NULL	NULL	0	NULL	Iron ( Fe )	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Four coastal Aboriginal settlements in the northwest area of Australia have been investigated for plasma trace metal status -- Zinc ( Zn ) , Copper ( Cu ) , and Iron ( Fe ) .
	manualset3
230865	1	428053	15	NULL	NULL	0	NULL	Four compounds 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four compounds of the ellipticine family were examined in their interaction with liposomes and with an isolated bacterial membrane .
	manualset3
230903	2	428053	15	NULL	NULL	0	NULL	ellipticine family	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Four compounds of the ellipticine family were examined in their interaction with liposomes and with an isolated bacterial membrane .
	manualset3
230904	3	428053	15	NULL	NULL	0	NULL	interaction	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Four compounds of the ellipticine family were examined in their interaction with liposomes and with an isolated bacterial membrane .
	manualset3
231074	4	428053	15	NULL	NULL	0	NULL	liposomes	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Four compounds of the ellipticine family were examined in their interaction with liposomes and with an isolated bacterial membrane .
	manualset3
231080	5	428053	15	NULL	NULL	0	NULL	isolated bacterial membrane	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Four compounds of the ellipticine family were examined in their interaction with liposomes and with an isolated bacterial membrane .
	manualset3
230893	2	428054	15	NULL	NULL	NULL	NULL	fixation/permeabilization	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four currently utilized procedures for fixation/permeabilization of intracellular antigens were compared for their ability to stain the nuclear antigens .
	manualset3
230897	3	428054	15	NULL	NULL	NULL	NULL	intracellular antigens	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four currently utilized procedures for fixation/permeabilization of intracellular antigens were compared for their ability to stain the nuclear antigens .
	manualset3
230899	4	428054	15	NULL	NULL	NULL	NULL	ability	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four currently utilized procedures for fixation/permeabilization of intracellular antigens were compared for their ability to stain the nuclear antigens .
	manualset3
230900	5	428054	15	NULL	NULL	NULL	NULL	nuclear antigens	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four currently utilized procedures for fixation/permeabilization of intracellular antigens were compared for their ability to stain the nuclear antigens .
	manualset3
230901	1	428054	15	NULL	NULL	NULL	NULL	Four currently utilized procedures	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four currently utilized procedures for fixation/permeabilization of intracellular antigens were compared for their ability to stain the nuclear antigens .
	manualset3
230902	1	428055	15	NULL	NULL	0	NULL	Four 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four different anti-CD5 mAb ( anti-Leu1 , 10.2 , anti-T1 , and OKT1 ) had a similar effect .
	manualset3
230905	2	428055	15	NULL	NULL	0	NULL	anti-CD5 mAb	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Four different anti-CD5 mAb ( anti-Leu1 , 10.2 , anti-T1 , and OKT1 ) had a similar effect .
	manualset3
230906	3	428055	15	NULL	NULL	0	NULL	anti-Leu1	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Four different anti-CD5 mAb ( anti-Leu1 , 10.2 , anti-T1 , and OKT1 ) had a similar effect .
	manualset3
230907	4	428055	15	NULL	NULL	0	NULL	10.2 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four different anti-CD5 mAb ( anti-Leu1 , 10.2 , anti-T1 , and OKT1 ) had a similar effect .
	manualset3
230908	5	428055	15	NULL	NULL	0	NULL	anti-T1	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Four different anti-CD5 mAb ( anti-Leu1 , 10.2 , anti-T1 , and OKT1 ) had a similar effect .
	manualset3
230909	6	428055	15	NULL	NULL	0	NULL	OKT1	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Four different anti-CD5 mAb ( anti-Leu1 , 10.2 , anti-T1 , and OKT1 ) had a similar effect .
	manualset3
230910	7	428055	15	NULL	NULL	0	NULL	effect	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Four different anti-CD5 mAb ( anti-Leu1 , 10.2 , anti-T1 , and OKT1 ) had a similar effect .
	manualset3
231082	1	428056	15	NULL	NULL	0	NULL	Four 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four different regimes of deformation are characterized as these parameters are systematically varied : ( i ) small deformation regime , ( ii ) disk formation regime , ( iii ) isotropic buckling regime , and ( iv ) anisotropic buckling regime .
	manualset3
231085	2	428056	15	NULL	NULL	0	NULL	regimes of deformation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Four different regimes of deformation are characterized as these parameters are systematically varied : ( i ) small deformation regime , ( ii ) disk formation regime , ( iii ) isotropic buckling regime , and ( iv ) anisotropic buckling regime .
	manualset3
231090	3	428056	15	NULL	NULL	0	NULL	parameters	ExperimentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Four different regimes of deformation are characterized as these parameters are systematically varied : ( i ) small deformation regime , ( ii ) disk formation regime , ( iii ) isotropic buckling regime , and ( iv ) anisotropic buckling regime .
	manualset3
231091	4	428056	15	NULL	NULL	NULL	NULL	small deformation regime	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four different regimes of deformation are characterized as these parameters are systematically varied : ( i ) small deformation regime , ( ii ) disk formation regime , ( iii ) isotropic buckling regime , and ( iv ) anisotropic buckling regime .
	manualset3
231092	5	428056	15	NULL	NULL	NULL	NULL	disk formation regime	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four different regimes of deformation are characterized as these parameters are systematically varied : ( i ) small deformation regime , ( ii ) disk formation regime , ( iii ) isotropic buckling regime , and ( iv ) anisotropic buckling regime .
	manualset3
231093	6	428056	15	NULL	NULL	NULL	NULL	isotropic buckling regime	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four different regimes of deformation are characterized as these parameters are systematically varied : ( i ) small deformation regime , ( ii ) disk formation regime , ( iii ) isotropic buckling regime , and ( iv ) anisotropic buckling regime .
	manualset3
231094	7	428056	15	NULL	NULL	NULL	NULL	anisotropic buckling regime	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four different regimes of deformation are characterized as these parameters are systematically varied : ( i ) small deformation regime , ( ii ) disk formation regime , ( iii ) isotropic buckling regime , and ( iv ) anisotropic buckling regime .
	manualset3
231095	1	428057	15	NULL	NULL	0	NULL	Four	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four distinct K + currents have been identified in Drosophila larval muscle fibers , i.e. the voltage-activated transient IA and delayed IK and the Ca ( 2 + ) - activated fast ICF and slow ICS .
	manualset3
231096	2	428057	15	NULL	NULL	0	NULL	K + currents	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Four distinct K + currents have been identified in Drosophila larval muscle fibers , i.e. the voltage-activated transient IA and delayed IK and the Ca ( 2 + ) - activated fast ICF and slow ICS .
	manualset3
231098	3	428057	15	NULL	NULL	0	NULL	Drosophila larval muscle fibers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Four distinct K + currents have been identified in Drosophila larval muscle fibers , i.e. the voltage-activated transient IA and delayed IK and the Ca ( 2 + ) - activated fast ICF and slow ICS .
	manualset3
231100	4	428057	15	NULL	NULL	0	NULL	voltage-activated transient IA	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Four distinct K + currents have been identified in Drosophila larval muscle fibers , i.e. the voltage-activated transient IA and delayed IK and the Ca ( 2 + ) - activated fast ICF and slow ICS .
	manualset3
231101	5	428057	15	NULL	NULL	0	NULL	delayed IK	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Four distinct K + currents have been identified in Drosophila larval muscle fibers , i.e. the voltage-activated transient IA and delayed IK and the Ca ( 2 + ) - activated fast ICF and slow ICS .
	manualset3
231102	6	428057	15	NULL	NULL	0	NULL	Ca ( 2 + ) - activated fast ICF	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Four distinct K + currents have been identified in Drosophila larval muscle fibers , i.e. the voltage-activated transient IA and delayed IK and the Ca ( 2 + ) - activated fast ICF and slow ICS .
	manualset3
231103	7	428057	15	NULL	NULL	0	NULL	slow ICS	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Four distinct K + currents have been identified in Drosophila larval muscle fibers , i.e. the voltage-activated transient IA and delayed IK and the Ca ( 2 + ) - activated fast ICF and slow ICS .
	manualset3
231104	1	428058	15	NULL	NULL	0	NULL	Research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Research on vaginal smears in the course of the estrus cycle in the guinea pig ) .
	manualset3
231105	2	428058	15	NULL	NULL	NULL	NULL	vaginal smears	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Research on vaginal smears in the course of the estrus cycle in the guinea pig ) .
	manualset3
231106	3	428058	15	NULL	NULL	0	NULL	course	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Research on vaginal smears in the course of the estrus cycle in the guinea pig ) .
	manualset3
231107	4	428058	15	NULL	NULL	0	NULL	estrus cycle	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	( Research on vaginal smears in the course of the estrus cycle in the guinea pig ) .
	manualset3
231108	5	428058	15	NULL	NULL	0	NULL	guinea pig	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	( Research on vaginal smears in the course of the estrus cycle in the guinea pig ) .
	manualset3
231109	1	428059	15	NULL	NULL	0	NULL	Four experimental scenarios	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four experimental scenarios of increasing complexity empirically demonstrate that this trace particulate evidence exhibits behavior in accordance with that previously identified for hair and fiber evidence .
	manualset3
231111	2	428059	15	NULL	NULL	0	NULL	complexity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Four experimental scenarios of increasing complexity empirically demonstrate that this trace particulate evidence exhibits behavior in accordance with that previously identified for hair and fiber evidence .
	manualset3
231113	3	428059	15	NULL	NULL	NULL	NULL	trace	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four experimental scenarios of increasing complexity empirically demonstrate that this trace particulate evidence exhibits behavior in accordance with that previously identified for hair and fiber evidence .
	manualset3
231115	5	428059	15	NULL	NULL	NULL	NULL	behavior	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four experimental scenarios of increasing complexity empirically demonstrate that this trace particulate evidence exhibits behavior in accordance with that previously identified for hair and fiber evidence .
	manualset3
231116	6	428059	15	NULL	NULL	NULL	NULL	accordance	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four experimental scenarios of increasing complexity empirically demonstrate that this trace particulate evidence exhibits behavior in accordance with that previously identified for hair and fiber evidence .
	manualset3
231117	7	428059	15	NULL	NULL	NULL	NULL	hair	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four experimental scenarios of increasing complexity empirically demonstrate that this trace particulate evidence exhibits behavior in accordance with that previously identified for hair and fiber evidence .
	manualset3
231118	8	428059	15	NULL	NULL	NULL	NULL	fiber evidence	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four experimental scenarios of increasing complexity empirically demonstrate that this trace particulate evidence exhibits behavior in accordance with that previously identified for hair and fiber evidence .
	manualset3
231533	4	428059	15	NULL	NULL	NULL	NULL	particulate evidence	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four experimental scenarios of increasing complexity empirically demonstrate that this trace particulate evidence exhibits behavior in accordance with that previously identified for hair and fiber evidence .
	manualset3
231119	1	428060	15	NULL	NULL	0	NULL	Four formulations	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four formulations were tested : a nanosuspension type DissoCube ( R ) , one solid lipid nanoparticle ( SLN ) preparation and two suspensions of micronized fenofibrate as reference formulations , one suspension in sirupus simplex and a second in a solution of hydroxyethy-cellulose in physiological saline .
	manualset3
231120	2	428060	15	NULL	NULL	NULL	NULL	nanosuspension type DissoCube ( R )	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four formulations were tested : a nanosuspension type DissoCube ( R ) , one solid lipid nanoparticle ( SLN ) preparation and two suspensions of micronized fenofibrate as reference formulations , one suspension in sirupus simplex and a second in a solution of hydroxyethy-cellulose in physiological saline .
	manualset3
231121	3	428060	15	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four formulations were tested : a nanosuspension type DissoCube ( R ) , one solid lipid nanoparticle ( SLN ) preparation and two suspensions of micronized fenofibrate as reference formulations , one suspension in sirupus simplex and a second in a solution of hydroxyethy-cellulose in physiological saline .
	manualset3
231122	4	428060	15	NULL	NULL	NULL	NULL	solid lipid nanoparticle ( SLN ) preparation	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four formulations were tested : a nanosuspension type DissoCube ( R ) , one solid lipid nanoparticle ( SLN ) preparation and two suspensions of micronized fenofibrate as reference formulations , one suspension in sirupus simplex and a second in a solution of hydroxyethy-cellulose in physiological saline .
	manualset3
231123	5	428060	15	NULL	NULL	0	NULL	two 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four formulations were tested : a nanosuspension type DissoCube ( R ) , one solid lipid nanoparticle ( SLN ) preparation and two suspensions of micronized fenofibrate as reference formulations , one suspension in sirupus simplex and a second in a solution of hydroxyethy-cellulose in physiological saline .
	manualset3
231124	6	428060	15	NULL	NULL	NULL	NULL	suspensions of micronized fenofibrate	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four formulations were tested : a nanosuspension type DissoCube ( R ) , one solid lipid nanoparticle ( SLN ) preparation and two suspensions of micronized fenofibrate as reference formulations , one suspension in sirupus simplex and a second in a solution of hydroxyethy-cellulose in physiological saline .
	manualset3
231125	7	428060	15	NULL	NULL	NULL	NULL	reference formulations	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four formulations were tested : a nanosuspension type DissoCube ( R ) , one solid lipid nanoparticle ( SLN ) preparation and two suspensions of micronized fenofibrate as reference formulations , one suspension in sirupus simplex and a second in a solution of hydroxyethy-cellulose in physiological saline .
	manualset3
231126	8	428060	15	NULL	NULL	NULL	NULL	one suspension	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four formulations were tested : a nanosuspension type DissoCube ( R ) , one solid lipid nanoparticle ( SLN ) preparation and two suspensions of micronized fenofibrate as reference formulations , one suspension in sirupus simplex and a second in a solution of hydroxyethy-cellulose in physiological saline .
	manualset3
231127	9	428060	15	NULL	NULL	0	NULL	sirupus simplex	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Four formulations were tested : a nanosuspension type DissoCube ( R ) , one solid lipid nanoparticle ( SLN ) preparation and two suspensions of micronized fenofibrate as reference formulations , one suspension in sirupus simplex and a second in a solution of hydroxyethy-cellulose in physiological saline .
	manualset3
231128	10	428060	15	NULL	NULL	0	NULL	solution of hydroxyethy-cellulose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Four formulations were tested : a nanosuspension type DissoCube ( R ) , one solid lipid nanoparticle ( SLN ) preparation and two suspensions of micronized fenofibrate as reference formulations , one suspension in sirupus simplex and a second in a solution of hydroxyethy-cellulose in physiological saline .
	manualset3
231129	11	428060	15	NULL	NULL	0	NULL	physiological saline	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Four formulations were tested : a nanosuspension type DissoCube ( R ) , one solid lipid nanoparticle ( SLN ) preparation and two suspensions of micronized fenofibrate as reference formulations , one suspension in sirupus simplex and a second in a solution of hydroxyethy-cellulose in physiological saline .
	manualset3
231136	1	428061	15	NULL	NULL	0	NULL	Four full-length cDNA clones	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four full-length cDNA clones coding for preprocathepsin B were isolated from a human gastric adenocarcinoma cDNA library ( AGS 1-6-30-1 ) and analyzed for possible sequence modifications that might be linked to altered intracellular trafficking and secretion of cathepsin B ( CTSB ) in malignant tumors .
	manualset3
231137	2	428061	15	NULL	NULL	0	NULL	preprocathepsin B	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Four full-length cDNA clones coding for preprocathepsin B were isolated from a human gastric adenocarcinoma cDNA library ( AGS 1-6-30-1 ) and analyzed for possible sequence modifications that might be linked to altered intracellular trafficking and secretion of cathepsin B ( CTSB ) in malignant tumors .
	manualset3
231140	3	428061	15	NULL	NULL	NULL	NULL	human gastric adenocarcinoma cDNA library ( AGS 1-6-30-1 )	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four full-length cDNA clones coding for preprocathepsin B were isolated from a human gastric adenocarcinoma cDNA library ( AGS 1-6-30-1 ) and analyzed for possible sequence modifications that might be linked to altered intracellular trafficking and secretion of cathepsin B ( CTSB ) in malignant tumors .
	manualset3
231143	4	428061	15	NULL	NULL	0	NULL	sequence modifications	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Four full-length cDNA clones coding for preprocathepsin B were isolated from a human gastric adenocarcinoma cDNA library ( AGS 1-6-30-1 ) and analyzed for possible sequence modifications that might be linked to altered intracellular trafficking and secretion of cathepsin B ( CTSB ) in malignant tumors .
	manualset3
231146	5	428061	15	NULL	NULL	NULL	NULL	intracellular trafficking	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four full-length cDNA clones coding for preprocathepsin B were isolated from a human gastric adenocarcinoma cDNA library ( AGS 1-6-30-1 ) and analyzed for possible sequence modifications that might be linked to altered intracellular trafficking and secretion of cathepsin B ( CTSB ) in malignant tumors .
	manualset3
231156	6	428061	15	NULL	NULL	NULL	NULL	secretion of cathepsin B ( CTSB )	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four full-length cDNA clones coding for preprocathepsin B were isolated from a human gastric adenocarcinoma cDNA library ( AGS 1-6-30-1 ) and analyzed for possible sequence modifications that might be linked to altered intracellular trafficking and secretion of cathepsin B ( CTSB ) in malignant tumors .
	manualset3
231160	7	428061	15	NULL	NULL	NULL	NULL	malignant tumors	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four full-length cDNA clones coding for preprocathepsin B were isolated from a human gastric adenocarcinoma cDNA library ( AGS 1-6-30-1 ) and analyzed for possible sequence modifications that might be linked to altered intracellular trafficking and secretion of cathepsin B ( CTSB ) in malignant tumors .
	manualset3
231165	1	428062	15	NULL	NULL	0	NULL	Four	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four fundamental principles of medical globalization emerged from in-depth interviews and analysis of observational materials : ( 1 ) the notion of history as an autonomous force with globalization as the latest stage , ( 2 ) the expansion of ` Total Market ' philosophy as a driving social force , ( 3 ) the fragmentation of society into atomistic , self-interested , and competitive individuals , and ( 4 ) the adoption of a ` centralised ' set of ideals as the normative core necessary for social order .
	manualset3
231168	2	428062	15	NULL	NULL	0	NULL	fundamental principles of medical globalization	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Four fundamental principles of medical globalization emerged from in-depth interviews and analysis of observational materials : ( 1 ) the notion of history as an autonomous force with globalization as the latest stage , ( 2 ) the expansion of ` Total Market ' philosophy as a driving social force , ( 3 ) the fragmentation of society into atomistic , self-interested , and competitive individuals , and ( 4 ) the adoption of a ` centralised ' set of ideals as the normative core necessary for social order .
	manualset3
231256	3	428062	15	NULL	NULL	0	NULL	interviews	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Four fundamental principles of medical globalization emerged from in-depth interviews and analysis of observational materials : ( 1 ) the notion of history as an autonomous force with globalization as the latest stage , ( 2 ) the expansion of ` Total Market ' philosophy as a driving social force , ( 3 ) the fragmentation of society into atomistic , self-interested , and competitive individuals , and ( 4 ) the adoption of a ` centralised ' set of ideals as the normative core necessary for social order .
	manualset3
231257	4	428062	15	NULL	NULL	0	NULL	analysis of observational materials	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four fundamental principles of medical globalization emerged from in-depth interviews and analysis of observational materials : ( 1 ) the notion of history as an autonomous force with globalization as the latest stage , ( 2 ) the expansion of ` Total Market ' philosophy as a driving social force , ( 3 ) the fragmentation of society into atomistic , self-interested , and competitive individuals , and ( 4 ) the adoption of a ` centralised ' set of ideals as the normative core necessary for social order .
	manualset3
231258	5	428062	15	NULL	NULL	0	NULL	notion	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Four fundamental principles of medical globalization emerged from in-depth interviews and analysis of observational materials : ( 1 ) the notion of history as an autonomous force with globalization as the latest stage , ( 2 ) the expansion of ` Total Market ' philosophy as a driving social force , ( 3 ) the fragmentation of society into atomistic , self-interested , and competitive individuals , and ( 4 ) the adoption of a ` centralised ' set of ideals as the normative core necessary for social order .
	manualset3
231259	6	428062	15	NULL	NULL	0	NULL	history	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Four fundamental principles of medical globalization emerged from in-depth interviews and analysis of observational materials : ( 1 ) the notion of history as an autonomous force with globalization as the latest stage , ( 2 ) the expansion of ` Total Market ' philosophy as a driving social force , ( 3 ) the fragmentation of society into atomistic , self-interested , and competitive individuals , and ( 4 ) the adoption of a ` centralised ' set of ideals as the normative core necessary for social order .
	manualset3
231260	7	428062	15	NULL	NULL	0	NULL	autonomous force	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Four fundamental principles of medical globalization emerged from in-depth interviews and analysis of observational materials : ( 1 ) the notion of history as an autonomous force with globalization as the latest stage , ( 2 ) the expansion of ` Total Market ' philosophy as a driving social force , ( 3 ) the fragmentation of society into atomistic , self-interested , and competitive individuals , and ( 4 ) the adoption of a ` centralised ' set of ideals as the normative core necessary for social order .
	manualset3
231261	8	428062	15	NULL	NULL	0	NULL	globalization 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Four fundamental principles of medical globalization emerged from in-depth interviews and analysis of observational materials : ( 1 ) the notion of history as an autonomous force with globalization as the latest stage , ( 2 ) the expansion of ` Total Market ' philosophy as a driving social force , ( 3 ) the fragmentation of society into atomistic , self-interested , and competitive individuals , and ( 4 ) the adoption of a ` centralised ' set of ideals as the normative core necessary for social order .
	manualset3
231270	9	428062	15	NULL	NULL	0	NULL	latest stage	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Four fundamental principles of medical globalization emerged from in-depth interviews and analysis of observational materials : ( 1 ) the notion of history as an autonomous force with globalization as the latest stage , ( 2 ) the expansion of ` Total Market ' philosophy as a driving social force , ( 3 ) the fragmentation of society into atomistic , self-interested , and competitive individuals , and ( 4 ) the adoption of a ` centralised ' set of ideals as the normative core necessary for social order .
	manualset3
231271	10	428062	15	NULL	NULL	0	NULL	expansion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Four fundamental principles of medical globalization emerged from in-depth interviews and analysis of observational materials : ( 1 ) the notion of history as an autonomous force with globalization as the latest stage , ( 2 ) the expansion of ` Total Market ' philosophy as a driving social force , ( 3 ) the fragmentation of society into atomistic , self-interested , and competitive individuals , and ( 4 ) the adoption of a ` centralised ' set of ideals as the normative core necessary for social order .
	manualset3
231272	11	428062	15	NULL	NULL	0	NULL	` Total Market ' philosophy	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Four fundamental principles of medical globalization emerged from in-depth interviews and analysis of observational materials : ( 1 ) the notion of history as an autonomous force with globalization as the latest stage , ( 2 ) the expansion of ` Total Market ' philosophy as a driving social force , ( 3 ) the fragmentation of society into atomistic , self-interested , and competitive individuals , and ( 4 ) the adoption of a ` centralised ' set of ideals as the normative core necessary for social order .
	manualset3
231279	12	428062	15	NULL	NULL	0	NULL	social force	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Four fundamental principles of medical globalization emerged from in-depth interviews and analysis of observational materials : ( 1 ) the notion of history as an autonomous force with globalization as the latest stage , ( 2 ) the expansion of ` Total Market ' philosophy as a driving social force , ( 3 ) the fragmentation of society into atomistic , self-interested , and competitive individuals , and ( 4 ) the adoption of a ` centralised ' set of ideals as the normative core necessary for social order .
	manualset3
231280	13	428062	15	NULL	NULL	0	NULL	fragmentation of society	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Four fundamental principles of medical globalization emerged from in-depth interviews and analysis of observational materials : ( 1 ) the notion of history as an autonomous force with globalization as the latest stage , ( 2 ) the expansion of ` Total Market ' philosophy as a driving social force , ( 3 ) the fragmentation of society into atomistic , self-interested , and competitive individuals , and ( 4 ) the adoption of a ` centralised ' set of ideals as the normative core necessary for social order .
	manualset3
231281	14	428062	15	NULL	NULL	NULL	NULL	atomistic individuals	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four fundamental principles of medical globalization emerged from in-depth interviews and analysis of observational materials : ( 1 ) the notion of history as an autonomous force with globalization as the latest stage , ( 2 ) the expansion of ` Total Market ' philosophy as a driving social force , ( 3 ) the fragmentation of society into atomistic , self-interested , and competitive individuals , and ( 4 ) the adoption of a ` centralised ' set of ideals as the normative core necessary for social order .
	manualset3
231282	15	428062	15	NULL	NULL	NULL	NULL	self-interested individuals	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four fundamental principles of medical globalization emerged from in-depth interviews and analysis of observational materials : ( 1 ) the notion of history as an autonomous force with globalization as the latest stage , ( 2 ) the expansion of ` Total Market ' philosophy as a driving social force , ( 3 ) the fragmentation of society into atomistic , self-interested , and competitive individuals , and ( 4 ) the adoption of a ` centralised ' set of ideals as the normative core necessary for social order .
	manualset3
231283	16	428062	15	NULL	NULL	0	NULL	competitive individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Four fundamental principles of medical globalization emerged from in-depth interviews and analysis of observational materials : ( 1 ) the notion of history as an autonomous force with globalization as the latest stage , ( 2 ) the expansion of ` Total Market ' philosophy as a driving social force , ( 3 ) the fragmentation of society into atomistic , self-interested , and competitive individuals , and ( 4 ) the adoption of a ` centralised ' set of ideals as the normative core necessary for social order .
	manualset3
231284	17	428062	15	NULL	NULL	0	NULL	adoption	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Four fundamental principles of medical globalization emerged from in-depth interviews and analysis of observational materials : ( 1 ) the notion of history as an autonomous force with globalization as the latest stage , ( 2 ) the expansion of ` Total Market ' philosophy as a driving social force , ( 3 ) the fragmentation of society into atomistic , self-interested , and competitive individuals , and ( 4 ) the adoption of a ` centralised ' set of ideals as the normative core necessary for social order .
	manualset3
231285	18	428062	15	NULL	NULL	0	NULL	ideals 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Four fundamental principles of medical globalization emerged from in-depth interviews and analysis of observational materials : ( 1 ) the notion of history as an autonomous force with globalization as the latest stage , ( 2 ) the expansion of ` Total Market ' philosophy as a driving social force , ( 3 ) the fragmentation of society into atomistic , self-interested , and competitive individuals , and ( 4 ) the adoption of a ` centralised ' set of ideals as the normative core necessary for social order .
	manualset3
231286	19	428062	15	NULL	NULL	NULL	NULL	normative core 	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four fundamental principles of medical globalization emerged from in-depth interviews and analysis of observational materials : ( 1 ) the notion of history as an autonomous force with globalization as the latest stage , ( 2 ) the expansion of ` Total Market ' philosophy as a driving social force , ( 3 ) the fragmentation of society into atomistic , self-interested , and competitive individuals , and ( 4 ) the adoption of a ` centralised ' set of ideals as the normative core necessary for social order .
	manualset3
231287	20	428062	15	NULL	NULL	0	NULL	social order	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Four fundamental principles of medical globalization emerged from in-depth interviews and analysis of observational materials : ( 1 ) the notion of history as an autonomous force with globalization as the latest stage , ( 2 ) the expansion of ` Total Market ' philosophy as a driving social force , ( 3 ) the fragmentation of society into atomistic , self-interested , and competitive individuals , and ( 4 ) the adoption of a ` centralised ' set of ideals as the normative core necessary for social order .
	manualset3
231189	1	428063	15	NULL	NULL	0	NULL	Four 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four gated SPECT slices were obtained on mid-ventricular vertical long axis , horizontal long axis and apical and basal short axis planes , and displayed in cine-format .
	manualset3
231190	2	428063	15	NULL	NULL	0	NULL	gated SPECT slices	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Four gated SPECT slices were obtained on mid-ventricular vertical long axis , horizontal long axis and apical and basal short axis planes , and displayed in cine-format .
	manualset3
231292	3	428063	15	NULL	NULL	0	NULL	mid-ventricular vertical long axis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Four gated SPECT slices were obtained on mid-ventricular vertical long axis , horizontal long axis and apical and basal short axis planes , and displayed in cine-format .
	manualset3
231293	4	428063	15	NULL	NULL	0	NULL	horizontal long axis	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Four gated SPECT slices were obtained on mid-ventricular vertical long axis , horizontal long axis and apical and basal short axis planes , and displayed in cine-format .
	manualset3
231294	5	428063	15	NULL	NULL	NULL	NULL	apical short axis plane	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four gated SPECT slices were obtained on mid-ventricular vertical long axis , horizontal long axis and apical and basal short axis planes , and displayed in cine-format .
	manualset3
231296	7	428063	15	NULL	NULL	NULL	NULL	cine-format	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four gated SPECT slices were obtained on mid-ventricular vertical long axis , horizontal long axis and apical and basal short axis planes , and displayed in cine-format .
	manualset3
231968	6	428063	15	NULL	NULL	0	NULL	basal short axis plane	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Four gated SPECT slices were obtained on mid-ventricular vertical long axis , horizontal long axis and apical and basal short axis planes , and displayed in cine-format .
	manualset3
231191	1	428064	15	NULL	NULL	NULL	NULL	Four generations	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four generations of dihydropyridines are now available .
	manualset3
231192	2	428064	15	NULL	NULL	0	NULL	dihydropyridines	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Four generations of dihydropyridines are now available .
	manualset3
231193	1	428065	15	NULL	NULL	0	NULL	Four groups	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four groups were studied : ( 1 ) Individuals with chronic asymptomatic infection with a positive test for IgG anti-Toxoplasma and without ocular lesions ( n = 16 ) ; ( 2 ) Chronic asymptomatic patients with retinal scars of retinochoroiditis by Toxoplasma ( n = 19 ) ; ( 3 ) Acute symptomatic patients with active retinochoroiditis by Toxoplasma ( n = 26 ) ; ( 4 ) Individuals with negative assays for IgG anti-Toxoplasma ( n = 21 ) .
	manualset3
231194	2	428065	15	NULL	NULL	0	NULL	Individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Four groups were studied : ( 1 ) Individuals with chronic asymptomatic infection with a positive test for IgG anti-Toxoplasma and without ocular lesions ( n = 16 ) ; ( 2 ) Chronic asymptomatic patients with retinal scars of retinochoroiditis by Toxoplasma ( n = 19 ) ; ( 3 ) Acute symptomatic patients with active retinochoroiditis by Toxoplasma ( n = 26 ) ; ( 4 ) Individuals with negative assays for IgG anti-Toxoplasma ( n = 21 ) .
	manualset3
231195	3	428065	15	NULL	NULL	0	NULL	chronic asymptomatic infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Four groups were studied : ( 1 ) Individuals with chronic asymptomatic infection with a positive test for IgG anti-Toxoplasma and without ocular lesions ( n = 16 ) ; ( 2 ) Chronic asymptomatic patients with retinal scars of retinochoroiditis by Toxoplasma ( n = 19 ) ; ( 3 ) Acute symptomatic patients with active retinochoroiditis by Toxoplasma ( n = 26 ) ; ( 4 ) Individuals with negative assays for IgG anti-Toxoplasma ( n = 21 ) .
	manualset3
231196	4	428065	15	NULL	NULL	NULL	NULL	positive test	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four groups were studied : ( 1 ) Individuals with chronic asymptomatic infection with a positive test for IgG anti-Toxoplasma and without ocular lesions ( n = 16 ) ; ( 2 ) Chronic asymptomatic patients with retinal scars of retinochoroiditis by Toxoplasma ( n = 19 ) ; ( 3 ) Acute symptomatic patients with active retinochoroiditis by Toxoplasma ( n = 26 ) ; ( 4 ) Individuals with negative assays for IgG anti-Toxoplasma ( n = 21 ) .
	manualset3
231197	5	428065	15	NULL	NULL	0	NULL	IgG anti-Toxoplasma	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Four groups were studied : ( 1 ) Individuals with chronic asymptomatic infection with a positive test for IgG anti-Toxoplasma and without ocular lesions ( n = 16 ) ; ( 2 ) Chronic asymptomatic patients with retinal scars of retinochoroiditis by Toxoplasma ( n = 19 ) ; ( 3 ) Acute symptomatic patients with active retinochoroiditis by Toxoplasma ( n = 26 ) ; ( 4 ) Individuals with negative assays for IgG anti-Toxoplasma ( n = 21 ) .
	manualset3
231198	6	428065	15	NULL	NULL	0	NULL	ocular lesions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Four groups were studied : ( 1 ) Individuals with chronic asymptomatic infection with a positive test for IgG anti-Toxoplasma and without ocular lesions ( n = 16 ) ; ( 2 ) Chronic asymptomatic patients with retinal scars of retinochoroiditis by Toxoplasma ( n = 19 ) ; ( 3 ) Acute symptomatic patients with active retinochoroiditis by Toxoplasma ( n = 26 ) ; ( 4 ) Individuals with negative assays for IgG anti-Toxoplasma ( n = 21 ) .
	manualset3
231199	7	428065	15	NULL	NULL	0	NULL	n = 16	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Four groups were studied : ( 1 ) Individuals with chronic asymptomatic infection with a positive test for IgG anti-Toxoplasma and without ocular lesions ( n = 16 ) ; ( 2 ) Chronic asymptomatic patients with retinal scars of retinochoroiditis by Toxoplasma ( n = 19 ) ; ( 3 ) Acute symptomatic patients with active retinochoroiditis by Toxoplasma ( n = 26 ) ; ( 4 ) Individuals with negative assays for IgG anti-Toxoplasma ( n = 21 ) .
	manualset3
231200	8	428065	15	NULL	NULL	0	NULL	Chronic asymptomatic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Four groups were studied : ( 1 ) Individuals with chronic asymptomatic infection with a positive test for IgG anti-Toxoplasma and without ocular lesions ( n = 16 ) ; ( 2 ) Chronic asymptomatic patients with retinal scars of retinochoroiditis by Toxoplasma ( n = 19 ) ; ( 3 ) Acute symptomatic patients with active retinochoroiditis by Toxoplasma ( n = 26 ) ; ( 4 ) Individuals with negative assays for IgG anti-Toxoplasma ( n = 21 ) .
	manualset3
231201	9	428065	15	NULL	NULL	0	NULL	retinal scars of retinochoroiditis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Four groups were studied : ( 1 ) Individuals with chronic asymptomatic infection with a positive test for IgG anti-Toxoplasma and without ocular lesions ( n = 16 ) ; ( 2 ) Chronic asymptomatic patients with retinal scars of retinochoroiditis by Toxoplasma ( n = 19 ) ; ( 3 ) Acute symptomatic patients with active retinochoroiditis by Toxoplasma ( n = 26 ) ; ( 4 ) Individuals with negative assays for IgG anti-Toxoplasma ( n = 21 ) .
	manualset3
231202	10	428065	15	NULL	NULL	0	NULL	Toxoplasma	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Four groups were studied : ( 1 ) Individuals with chronic asymptomatic infection with a positive test for IgG anti-Toxoplasma and without ocular lesions ( n = 16 ) ; ( 2 ) Chronic asymptomatic patients with retinal scars of retinochoroiditis by Toxoplasma ( n = 19 ) ; ( 3 ) Acute symptomatic patients with active retinochoroiditis by Toxoplasma ( n = 26 ) ; ( 4 ) Individuals with negative assays for IgG anti-Toxoplasma ( n = 21 ) .
	manualset3
231203	11	428065	15	NULL	NULL	0	NULL	n = 19	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Four groups were studied : ( 1 ) Individuals with chronic asymptomatic infection with a positive test for IgG anti-Toxoplasma and without ocular lesions ( n = 16 ) ; ( 2 ) Chronic asymptomatic patients with retinal scars of retinochoroiditis by Toxoplasma ( n = 19 ) ; ( 3 ) Acute symptomatic patients with active retinochoroiditis by Toxoplasma ( n = 26 ) ; ( 4 ) Individuals with negative assays for IgG anti-Toxoplasma ( n = 21 ) .
	manualset3
231204	12	428065	15	NULL	NULL	NULL	NULL	Acute symptomatic patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four groups were studied : ( 1 ) Individuals with chronic asymptomatic infection with a positive test for IgG anti-Toxoplasma and without ocular lesions ( n = 16 ) ; ( 2 ) Chronic asymptomatic patients with retinal scars of retinochoroiditis by Toxoplasma ( n = 19 ) ; ( 3 ) Acute symptomatic patients with active retinochoroiditis by Toxoplasma ( n = 26 ) ; ( 4 ) Individuals with negative assays for IgG anti-Toxoplasma ( n = 21 ) .
	manualset3
231205	13	428065	15	NULL	NULL	0	NULL	active retinochoroiditis 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Four groups were studied : ( 1 ) Individuals with chronic asymptomatic infection with a positive test for IgG anti-Toxoplasma and without ocular lesions ( n = 16 ) ; ( 2 ) Chronic asymptomatic patients with retinal scars of retinochoroiditis by Toxoplasma ( n = 19 ) ; ( 3 ) Acute symptomatic patients with active retinochoroiditis by Toxoplasma ( n = 26 ) ; ( 4 ) Individuals with negative assays for IgG anti-Toxoplasma ( n = 21 ) .
	manualset3
231206	14	428065	15	NULL	NULL	0	NULL	Toxoplasma	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Four groups were studied : ( 1 ) Individuals with chronic asymptomatic infection with a positive test for IgG anti-Toxoplasma and without ocular lesions ( n = 16 ) ; ( 2 ) Chronic asymptomatic patients with retinal scars of retinochoroiditis by Toxoplasma ( n = 19 ) ; ( 3 ) Acute symptomatic patients with active retinochoroiditis by Toxoplasma ( n = 26 ) ; ( 4 ) Individuals with negative assays for IgG anti-Toxoplasma ( n = 21 ) .
	manualset3
231207	15	428065	15	NULL	NULL	0	NULL	 n = 26	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Four groups were studied : ( 1 ) Individuals with chronic asymptomatic infection with a positive test for IgG anti-Toxoplasma and without ocular lesions ( n = 16 ) ; ( 2 ) Chronic asymptomatic patients with retinal scars of retinochoroiditis by Toxoplasma ( n = 19 ) ; ( 3 ) Acute symptomatic patients with active retinochoroiditis by Toxoplasma ( n = 26 ) ; ( 4 ) Individuals with negative assays for IgG anti-Toxoplasma ( n = 21 ) .
	manualset3
231208	16	428065	15	NULL	NULL	0	NULL	Individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Four groups were studied : ( 1 ) Individuals with chronic asymptomatic infection with a positive test for IgG anti-Toxoplasma and without ocular lesions ( n = 16 ) ; ( 2 ) Chronic asymptomatic patients with retinal scars of retinochoroiditis by Toxoplasma ( n = 19 ) ; ( 3 ) Acute symptomatic patients with active retinochoroiditis by Toxoplasma ( n = 26 ) ; ( 4 ) Individuals with negative assays for IgG anti-Toxoplasma ( n = 21 ) .
	manualset3
231209	17	428065	15	NULL	NULL	NULL	NULL	negative assays	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four groups were studied : ( 1 ) Individuals with chronic asymptomatic infection with a positive test for IgG anti-Toxoplasma and without ocular lesions ( n = 16 ) ; ( 2 ) Chronic asymptomatic patients with retinal scars of retinochoroiditis by Toxoplasma ( n = 19 ) ; ( 3 ) Acute symptomatic patients with active retinochoroiditis by Toxoplasma ( n = 26 ) ; ( 4 ) Individuals with negative assays for IgG anti-Toxoplasma ( n = 21 ) .
	manualset3
231210	18	428065	15	NULL	NULL	0	NULL	IgG anti-Toxoplasma	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Four groups were studied : ( 1 ) Individuals with chronic asymptomatic infection with a positive test for IgG anti-Toxoplasma and without ocular lesions ( n = 16 ) ; ( 2 ) Chronic asymptomatic patients with retinal scars of retinochoroiditis by Toxoplasma ( n = 19 ) ; ( 3 ) Acute symptomatic patients with active retinochoroiditis by Toxoplasma ( n = 26 ) ; ( 4 ) Individuals with negative assays for IgG anti-Toxoplasma ( n = 21 ) .
	manualset3
231211	19	428065	15	NULL	NULL	0	NULL	 n = 21 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Four groups were studied : ( 1 ) Individuals with chronic asymptomatic infection with a positive test for IgG anti-Toxoplasma and without ocular lesions ( n = 16 ) ; ( 2 ) Chronic asymptomatic patients with retinal scars of retinochoroiditis by Toxoplasma ( n = 19 ) ; ( 3 ) Acute symptomatic patients with active retinochoroiditis by Toxoplasma ( n = 26 ) ; ( 4 ) Individuals with negative assays for IgG anti-Toxoplasma ( n = 21 ) .
	manualset3
231212	1	428066	15	NULL	NULL	0	NULL	Four	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four had meningoencephalitis , one meningeal and subcortical sarcoidosis nodules , four meningeal malignancies -- one disseminated oligodendroglioma , one with meningeal infiltration around an adenocarcinoma , three meningeal infiltration by a hematological malignancy , and one a chronic subdural hematoma without a history of injury .
	manualset3
231213	2	428066	15	NULL	NULL	0	NULL	meningoencephalitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Four had meningoencephalitis , one meningeal and subcortical sarcoidosis nodules , four meningeal malignancies -- one disseminated oligodendroglioma , one with meningeal infiltration around an adenocarcinoma , three meningeal infiltration by a hematological malignancy , and one a chronic subdural hematoma without a history of injury .
	manualset3
231214	3	428066	15	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four had meningoencephalitis , one meningeal and subcortical sarcoidosis nodules , four meningeal malignancies -- one disseminated oligodendroglioma , one with meningeal infiltration around an adenocarcinoma , three meningeal infiltration by a hematological malignancy , and one a chronic subdural hematoma without a history of injury .
	manualset3
231215	4	428066	15	NULL	NULL	NULL	NULL	meningeal nodule	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four had meningoencephalitis , one meningeal and subcortical sarcoidosis nodules , four meningeal malignancies -- one disseminated oligodendroglioma , one with meningeal infiltration around an adenocarcinoma , three meningeal infiltration by a hematological malignancy , and one a chronic subdural hematoma without a history of injury .
	manualset3
231216	6	428066	15	NULL	NULL	NULL	NULL	four	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four had meningoencephalitis , one meningeal and subcortical sarcoidosis nodules , four meningeal malignancies -- one disseminated oligodendroglioma , one with meningeal infiltration around an adenocarcinoma , three meningeal infiltration by a hematological malignancy , and one a chronic subdural hematoma without a history of injury .
	manualset3
231217	7	428066	15	NULL	NULL	NULL	NULL	meningeal malignancies	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four had meningoencephalitis , one meningeal and subcortical sarcoidosis nodules , four meningeal malignancies -- one disseminated oligodendroglioma , one with meningeal infiltration around an adenocarcinoma , three meningeal infiltration by a hematological malignancy , and one a chronic subdural hematoma without a history of injury .
	manualset3
231218	8	428066	15	NULL	NULL	NULL	NULL	one	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four had meningoencephalitis , one meningeal and subcortical sarcoidosis nodules , four meningeal malignancies -- one disseminated oligodendroglioma , one with meningeal infiltration around an adenocarcinoma , three meningeal infiltration by a hematological malignancy , and one a chronic subdural hematoma without a history of injury .
	manualset3
231219	9	428066	15	NULL	NULL	NULL	NULL	oligodendroglioma	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four had meningoencephalitis , one meningeal and subcortical sarcoidosis nodules , four meningeal malignancies -- one disseminated oligodendroglioma , one with meningeal infiltration around an adenocarcinoma , three meningeal infiltration by a hematological malignancy , and one a chronic subdural hematoma without a history of injury .
	manualset3
231220	10	428066	15	NULL	NULL	NULL	NULL	one	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four had meningoencephalitis , one meningeal and subcortical sarcoidosis nodules , four meningeal malignancies -- one disseminated oligodendroglioma , one with meningeal infiltration around an adenocarcinoma , three meningeal infiltration by a hematological malignancy , and one a chronic subdural hematoma without a history of injury .
	manualset3
231221	11	428066	15	NULL	NULL	NULL	NULL	meningeal infiltration	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four had meningoencephalitis , one meningeal and subcortical sarcoidosis nodules , four meningeal malignancies -- one disseminated oligodendroglioma , one with meningeal infiltration around an adenocarcinoma , three meningeal infiltration by a hematological malignancy , and one a chronic subdural hematoma without a history of injury .
	manualset3
231222	13	428066	15	NULL	NULL	NULL	NULL	three meningeal infiltration	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four had meningoencephalitis , one meningeal and subcortical sarcoidosis nodules , four meningeal malignancies -- one disseminated oligodendroglioma , one with meningeal infiltration around an adenocarcinoma , three meningeal infiltration by a hematological malignancy , and one a chronic subdural hematoma without a history of injury .
	manualset3
231249	14	428066	15	NULL	NULL	NULL	NULL	hematological malignancy	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four had meningoencephalitis , one meningeal and subcortical sarcoidosis nodules , four meningeal malignancies -- one disseminated oligodendroglioma , one with meningeal infiltration around an adenocarcinoma , three meningeal infiltration by a hematological malignancy , and one a chronic subdural hematoma without a history of injury .
	manualset3
231250	15	428066	15	NULL	NULL	NULL	NULL	one	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four had meningoencephalitis , one meningeal and subcortical sarcoidosis nodules , four meningeal malignancies -- one disseminated oligodendroglioma , one with meningeal infiltration around an adenocarcinoma , three meningeal infiltration by a hematological malignancy , and one a chronic subdural hematoma without a history of injury .
	manualset3
231251	16	428066	15	NULL	NULL	NULL	NULL	chronic subdural hematoma	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four had meningoencephalitis , one meningeal and subcortical sarcoidosis nodules , four meningeal malignancies -- one disseminated oligodendroglioma , one with meningeal infiltration around an adenocarcinoma , three meningeal infiltration by a hematological malignancy , and one a chronic subdural hematoma without a history of injury .
	manualset3
231252	17	428066	15	NULL	NULL	NULL	NULL	history	Time												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four had meningoencephalitis , one meningeal and subcortical sarcoidosis nodules , four meningeal malignancies -- one disseminated oligodendroglioma , one with meningeal infiltration around an adenocarcinoma , three meningeal infiltration by a hematological malignancy , and one a chronic subdural hematoma without a history of injury .
	manualset3
231253	18	428066	15	NULL	NULL	NULL	NULL	injury	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four had meningoencephalitis , one meningeal and subcortical sarcoidosis nodules , four meningeal malignancies -- one disseminated oligodendroglioma , one with meningeal infiltration around an adenocarcinoma , three meningeal infiltration by a hematological malignancy , and one a chronic subdural hematoma without a history of injury .
	manualset3
231969	5	428066	15	NULL	NULL	0	NULL	subcortical sarcoidosis nodule	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Four had meningoencephalitis , one meningeal and subcortical sarcoidosis nodules , four meningeal malignancies -- one disseminated oligodendroglioma , one with meningeal infiltration around an adenocarcinoma , three meningeal infiltration by a hematological malignancy , and one a chronic subdural hematoma without a history of injury .
	manualset3
231993	12	428066	15	NULL	NULL	0	NULL	adenocarcinoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Four had meningoencephalitis , one meningeal and subcortical sarcoidosis nodules , four meningeal malignancies -- one disseminated oligodendroglioma , one with meningeal infiltration around an adenocarcinoma , three meningeal infiltration by a hematological malignancy , and one a chronic subdural hematoma without a history of injury .
	manualset3
231254	1	428067	15	NULL	NULL	0	NULL	Four hundred and fifty-eight genes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four hundred and fifty-eight genes were characterized by higher rates of interstrain variation and were considered hyperdivergent .
	manualset3
231255	2	428067	15	NULL	NULL	NULL	NULL	higher rates	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four hundred and fifty-eight genes were characterized by higher rates of interstrain variation and were considered hyperdivergent .
	manualset3
231970	3	428067	15	NULL	NULL	0	NULL	interstrain variation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Four hundred and fifty-eight genes were characterized by higher rates of interstrain variation and were considered hyperdivergent .
	manualset3
231297	1	428068	15	NULL	NULL	0	NULL	Research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Research advances on RB1 gene ) .
	manualset3
231298	2	428068	15	NULL	NULL	0	NULL	advances	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Research advances on RB1 gene ) .
	manualset3
231299	3	428068	15	NULL	NULL	0	NULL	RB1 gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	( Research advances on RB1 gene ) .
	manualset3
231300	1	428069	15	NULL	NULL	0	NULL	Four issues	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four issues are identified as critical to this : theory-driven targets of public health significance , use of appropriate and sophisticated approaches to research design and statistical modeling , development of instruments and measures , and conclusions that make a difference .
	manualset3
231302	2	428069	15	NULL	NULL	NULL	NULL	theory-driven targets	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four issues are identified as critical to this : theory-driven targets of public health significance , use of appropriate and sophisticated approaches to research design and statistical modeling , development of instruments and measures , and conclusions that make a difference .
	manualset3
231307	6	428069	15	NULL	NULL	NULL	NULL	appropriate approaches	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four issues are identified as critical to this : theory-driven targets of public health significance , use of appropriate and sophisticated approaches to research design and statistical modeling , development of instruments and measures , and conclusions that make a difference .
	manualset3
231308	10	428069	15	NULL	NULL	NULL	NULL	development	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four issues are identified as critical to this : theory-driven targets of public health significance , use of appropriate and sophisticated approaches to research design and statistical modeling , development of instruments and measures , and conclusions that make a difference .
	manualset3
231309	13	428069	15	NULL	NULL	NULL	NULL	conclusions	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four issues are identified as critical to this : theory-driven targets of public health significance , use of appropriate and sophisticated approaches to research design and statistical modeling , development of instruments and measures , and conclusions that make a difference .
	manualset3
231310	14	428069	15	NULL	NULL	NULL	NULL	difference	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four issues are identified as critical to this : theory-driven targets of public health significance , use of appropriate and sophisticated approaches to research design and statistical modeling , development of instruments and measures , and conclusions that make a difference .
	manualset3
232003	4	428069	15	NULL	NULL	NULL	NULL	public health significance	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four issues are identified as critical to this : theory-driven targets of public health significance , use of appropriate and sophisticated approaches to research design and statistical modeling , development of instruments and measures , and conclusions that make a difference .
	manualset3
232004	7	428069	15	NULL	NULL	NULL	NULL	sophisticated approaches	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four issues are identified as critical to this : theory-driven targets of public health significance , use of appropriate and sophisticated approaches to research design and statistical modeling , development of instruments and measures , and conclusions that make a difference .
	manualset3
232015	11	428069	15	NULL	NULL	NULL	NULL	instruments	MedicalDevice												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four issues are identified as critical to this : theory-driven targets of public health significance , use of appropriate and sophisticated approaches to research design and statistical modeling , development of instruments and measures , and conclusions that make a difference .
	manualset3
232016	12	428069	15	NULL	NULL	NULL	NULL	measures	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four issues are identified as critical to this : theory-driven targets of public health significance , use of appropriate and sophisticated approaches to research design and statistical modeling , development of instruments and measures , and conclusions that make a difference .
	manualset3
234401	5	428069	15	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Four issues are identified as critical to this : theory-driven targets of public health significance , use of appropriate and sophisticated approaches to research design and statistical modeling , development of instruments and measures , and conclusions that make a difference .
	manualset3
234402	8	428069	15	NULL	NULL	0	NULL	research design	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Four issues are identified as critical to this : theory-driven targets of public health significance , use of appropriate and sophisticated approaches to research design and statistical modeling , development of instruments and measures , and conclusions that make a difference .
	manualset3
234403	9	428069	15	NULL	NULL	0	NULL	statistical modeling	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Four issues are identified as critical to this : theory-driven targets of public health significance , use of appropriate and sophisticated approaches to research design and statistical modeling , development of instruments and measures , and conclusions that make a difference .
	manualset3
231311	1	428070	15	NULL	NULL	0	NULL	Four loci	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four loci were represented by microsatellite polymorphisms and one ( GC ) was expressed as a protein polymorphism .
	manualset3
231312	2	428070	15	NULL	NULL	NULL	NULL	microsatellite polymorphisms	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four loci were represented by microsatellite polymorphisms and one ( GC ) was expressed as a protein polymorphism .
	manualset3
231417	3	428070	15	NULL	NULL	0	NULL	one ( GC )	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four loci were represented by microsatellite polymorphisms and one ( GC ) was expressed as a protein polymorphism .
	manualset3
231418	4	428070	15	NULL	NULL	0	NULL	protein polymorphism	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Four loci were represented by microsatellite polymorphisms and one ( GC ) was expressed as a protein polymorphism .
	manualset3
231552	1	428071	15	NULL	NULL	NULL	NULL	Four	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four nanofiltration and reverse osmosis membranes ( BW30 , ESPA4 , NF90 , TFC-S ) and a number of operation parameter combinations ( transmembrane pressure , feed flow , TFC-S ) and operating parameters transmembrane pressure and feed flow were investigated to find the best operating conditions for maximum drinking water production and minimum specific energy consumption ( SEC ) .
	manualset3
231555	3	428071	15	NULL	NULL	NULL	NULL	reverse osmosis membranes	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four nanofiltration and reverse osmosis membranes ( BW30 , ESPA4 , NF90 , TFC-S ) and a number of operation parameter combinations ( transmembrane pressure , feed flow , TFC-S ) and operating parameters transmembrane pressure and feed flow were investigated to find the best operating conditions for maximum drinking water production and minimum specific energy consumption ( SEC ) .
	manualset3
231556	4	428071	15	NULL	NULL	NULL	NULL	BW30	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four nanofiltration and reverse osmosis membranes ( BW30 , ESPA4 , NF90 , TFC-S ) and a number of operation parameter combinations ( transmembrane pressure , feed flow , TFC-S ) and operating parameters transmembrane pressure and feed flow were investigated to find the best operating conditions for maximum drinking water production and minimum specific energy consumption ( SEC ) .
	manualset3
231557	5	428071	15	NULL	NULL	NULL	NULL	ESPA4	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four nanofiltration and reverse osmosis membranes ( BW30 , ESPA4 , NF90 , TFC-S ) and a number of operation parameter combinations ( transmembrane pressure , feed flow , TFC-S ) and operating parameters transmembrane pressure and feed flow were investigated to find the best operating conditions for maximum drinking water production and minimum specific energy consumption ( SEC ) .
	manualset3
231558	6	428071	15	NULL	NULL	NULL	NULL	NF90	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four nanofiltration and reverse osmosis membranes ( BW30 , ESPA4 , NF90 , TFC-S ) and a number of operation parameter combinations ( transmembrane pressure , feed flow , TFC-S ) and operating parameters transmembrane pressure and feed flow were investigated to find the best operating conditions for maximum drinking water production and minimum specific energy consumption ( SEC ) .
	manualset3
231559	7	428071	15	NULL	NULL	NULL	NULL	TFC-S	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four nanofiltration and reverse osmosis membranes ( BW30 , ESPA4 , NF90 , TFC-S ) and a number of operation parameter combinations ( transmembrane pressure , feed flow , TFC-S ) and operating parameters transmembrane pressure and feed flow were investigated to find the best operating conditions for maximum drinking water production and minimum specific energy consumption ( SEC ) .
	manualset3
231560	8	428071	15	NULL	NULL	NULL	NULL	number 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four nanofiltration and reverse osmosis membranes ( BW30 , ESPA4 , NF90 , TFC-S ) and a number of operation parameter combinations ( transmembrane pressure , feed flow , TFC-S ) and operating parameters transmembrane pressure and feed flow were investigated to find the best operating conditions for maximum drinking water production and minimum specific energy consumption ( SEC ) .
	manualset3
231561	9	428071	15	NULL	NULL	NULL	NULL	operation parameter combinations	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four nanofiltration and reverse osmosis membranes ( BW30 , ESPA4 , NF90 , TFC-S ) and a number of operation parameter combinations ( transmembrane pressure , feed flow , TFC-S ) and operating parameters transmembrane pressure and feed flow were investigated to find the best operating conditions for maximum drinking water production and minimum specific energy consumption ( SEC ) .
	manualset3
231562	10	428071	15	NULL	NULL	NULL	NULL	transmembrane pressure	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four nanofiltration and reverse osmosis membranes ( BW30 , ESPA4 , NF90 , TFC-S ) and a number of operation parameter combinations ( transmembrane pressure , feed flow , TFC-S ) and operating parameters transmembrane pressure and feed flow were investigated to find the best operating conditions for maximum drinking water production and minimum specific energy consumption ( SEC ) .
	manualset3
231563	11	428071	15	NULL	NULL	NULL	NULL	feed flow	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four nanofiltration and reverse osmosis membranes ( BW30 , ESPA4 , NF90 , TFC-S ) and a number of operation parameter combinations ( transmembrane pressure , feed flow , TFC-S ) and operating parameters transmembrane pressure and feed flow were investigated to find the best operating conditions for maximum drinking water production and minimum specific energy consumption ( SEC ) .
	manualset3
231564	12	428071	15	NULL	NULL	NULL	NULL	TFC-S	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four nanofiltration and reverse osmosis membranes ( BW30 , ESPA4 , NF90 , TFC-S ) and a number of operation parameter combinations ( transmembrane pressure , feed flow , TFC-S ) and operating parameters transmembrane pressure and feed flow were investigated to find the best operating conditions for maximum drinking water production and minimum specific energy consumption ( SEC ) .
	manualset3
231569	13	428071	15	NULL	NULL	NULL	NULL	operating parameters	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four nanofiltration and reverse osmosis membranes ( BW30 , ESPA4 , NF90 , TFC-S ) and a number of operation parameter combinations ( transmembrane pressure , feed flow , TFC-S ) and operating parameters transmembrane pressure and feed flow were investigated to find the best operating conditions for maximum drinking water production and minimum specific energy consumption ( SEC ) .
	manualset3
231571	14	428071	15	NULL	NULL	NULL	NULL	transmembrane pressure 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four nanofiltration and reverse osmosis membranes ( BW30 , ESPA4 , NF90 , TFC-S ) and a number of operation parameter combinations ( transmembrane pressure , feed flow , TFC-S ) and operating parameters transmembrane pressure and feed flow were investigated to find the best operating conditions for maximum drinking water production and minimum specific energy consumption ( SEC ) .
	manualset3
231573	15	428071	15	NULL	NULL	NULL	NULL	feed flow	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four nanofiltration and reverse osmosis membranes ( BW30 , ESPA4 , NF90 , TFC-S ) and a number of operation parameter combinations ( transmembrane pressure , feed flow , TFC-S ) and operating parameters transmembrane pressure and feed flow were investigated to find the best operating conditions for maximum drinking water production and minimum specific energy consumption ( SEC ) .
	manualset3
231575	16	428071	15	NULL	NULL	NULL	NULL	operating conditions	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four nanofiltration and reverse osmosis membranes ( BW30 , ESPA4 , NF90 , TFC-S ) and a number of operation parameter combinations ( transmembrane pressure , feed flow , TFC-S ) and operating parameters transmembrane pressure and feed flow were investigated to find the best operating conditions for maximum drinking water production and minimum specific energy consumption ( SEC ) .
	manualset3
231577	17	428071	15	NULL	NULL	NULL	NULL	drinking water production	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four nanofiltration and reverse osmosis membranes ( BW30 , ESPA4 , NF90 , TFC-S ) and a number of operation parameter combinations ( transmembrane pressure , feed flow , TFC-S ) and operating parameters transmembrane pressure and feed flow were investigated to find the best operating conditions for maximum drinking water production and minimum specific energy consumption ( SEC ) .
	manualset3
231580	18	428071	15	NULL	NULL	NULL	NULL	specific energy consumption ( SEC )	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four nanofiltration and reverse osmosis membranes ( BW30 , ESPA4 , NF90 , TFC-S ) and a number of operation parameter combinations ( transmembrane pressure , feed flow , TFC-S ) and operating parameters transmembrane pressure and feed flow were investigated to find the best operating conditions for maximum drinking water production and minimum specific energy consumption ( SEC ) .
	manualset3
234404	2	428071	15	NULL	NULL	0	NULL	nanofiltration membranes	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Four nanofiltration and reverse osmosis membranes ( BW30 , ESPA4 , NF90 , TFC-S ) and a number of operation parameter combinations ( transmembrane pressure , feed flow , TFC-S ) and operating parameters transmembrane pressure and feed flow were investigated to find the best operating conditions for maximum drinking water production and minimum specific energy consumption ( SEC ) .
	manualset3
231581	1	428072	15	NULL	NULL	0	NULL	Research 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Research progress of diagnosis and treatment of Lisfrane injury ) .
	manualset3
231582	2	428072	15	NULL	NULL	0	NULL	progress	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Research progress of diagnosis and treatment of Lisfrane injury ) .
	manualset3
231584	3	428072	15	NULL	NULL	NULL	NULL	diagnosis	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Research progress of diagnosis and treatment of Lisfrane injury ) .
	manualset3
231586	4	428072	15	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Research progress of diagnosis and treatment of Lisfrane injury ) .
	manualset3
231587	5	428072	15	NULL	NULL	0	NULL	Lisfrane injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Research progress of diagnosis and treatment of Lisfrane injury ) .
	manualset3
231588	1	428073	15	NULL	NULL	0	NULL	Four of five social network indices	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four of five social network indices ( social anchorage , social participation , contact frequency , spousal support ) were associated with heavy drinking ( OR 1.9-2 .5 ) and two social network indices ( social anchorage , spousal support ) were associated with alcohol problems ( OR 2.1-2 .3 ) .
	manualset3
231590	2	428073	15	NULL	NULL	0	NULL	social anchorage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Four of five social network indices ( social anchorage , social participation , contact frequency , spousal support ) were associated with heavy drinking ( OR 1.9-2 .5 ) and two social network indices ( social anchorage , spousal support ) were associated with alcohol problems ( OR 2.1-2 .3 ) .
	manualset3
231591	3	428073	15	NULL	NULL	0	NULL	social participation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Four of five social network indices ( social anchorage , social participation , contact frequency , spousal support ) were associated with heavy drinking ( OR 1.9-2 .5 ) and two social network indices ( social anchorage , spousal support ) were associated with alcohol problems ( OR 2.1-2 .3 ) .
	manualset3
231594	4	428073	15	NULL	NULL	0	NULL	contact frequency	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Four of five social network indices ( social anchorage , social participation , contact frequency , spousal support ) were associated with heavy drinking ( OR 1.9-2 .5 ) and two social network indices ( social anchorage , spousal support ) were associated with alcohol problems ( OR 2.1-2 .3 ) .
	manualset3
231595	5	428073	15	NULL	NULL	0	NULL	spousal support	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Four of five social network indices ( social anchorage , social participation , contact frequency , spousal support ) were associated with heavy drinking ( OR 1.9-2 .5 ) and two social network indices ( social anchorage , spousal support ) were associated with alcohol problems ( OR 2.1-2 .3 ) .
	manualset3
231596	6	428073	15	NULL	NULL	0	NULL	( OR 1.9-2 .5 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Four of five social network indices ( social anchorage , social participation , contact frequency , spousal support ) were associated with heavy drinking ( OR 1.9-2 .5 ) and two social network indices ( social anchorage , spousal support ) were associated with alcohol problems ( OR 2.1-2 .3 ) .
	manualset3
231597	7	428073	15	NULL	NULL	0	NULL	two social network indices	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four of five social network indices ( social anchorage , social participation , contact frequency , spousal support ) were associated with heavy drinking ( OR 1.9-2 .5 ) and two social network indices ( social anchorage , spousal support ) were associated with alcohol problems ( OR 2.1-2 .3 ) .
	manualset3
231598	8	428073	15	NULL	NULL	0	NULL	social anchorage	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Four of five social network indices ( social anchorage , social participation , contact frequency , spousal support ) were associated with heavy drinking ( OR 1.9-2 .5 ) and two social network indices ( social anchorage , spousal support ) were associated with alcohol problems ( OR 2.1-2 .3 ) .
	manualset3
231600	9	428073	15	NULL	NULL	0	NULL	spousal support 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Four of five social network indices ( social anchorage , social participation , contact frequency , spousal support ) were associated with heavy drinking ( OR 1.9-2 .5 ) and two social network indices ( social anchorage , spousal support ) were associated with alcohol problems ( OR 2.1-2 .3 ) .
	manualset3
231604	10	428073	15	NULL	NULL	NULL	NULL	alcohol problems	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four of five social network indices ( social anchorage , social participation , contact frequency , spousal support ) were associated with heavy drinking ( OR 1.9-2 .5 ) and two social network indices ( social anchorage , spousal support ) were associated with alcohol problems ( OR 2.1-2 .3 ) .
	manualset3
231605	11	428073	15	NULL	NULL	0	NULL	( OR 2.1-2 .3 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Four of five social network indices ( social anchorage , social participation , contact frequency , spousal support ) were associated with heavy drinking ( OR 1.9-2 .5 ) and two social network indices ( social anchorage , spousal support ) were associated with alcohol problems ( OR 2.1-2 .3 ) .
	manualset3
231614	1	428074	15	NULL	NULL	0	NULL	Four polymorphs 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four polymorphs of IrI ( CO ) 2 ( OC ( CH3 ) CHC ( CH3 ) N ( p-tol ) ) have been characterized by single crystal X-ray crystallography .
	manualset3
231615	2	428074	15	NULL	NULL	0	NULL	IrI ( CO ) 2 ( OC ( CH3 ) CHC ( CH3 ) N ( p-tol ) )	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Four polymorphs of IrI ( CO ) 2 ( OC ( CH3 ) CHC ( CH3 ) N ( p-tol ) ) have been characterized by single crystal X-ray crystallography .
	manualset3
231616	3	428074	15	NULL	NULL	0	NULL	single crystal X-ray crystallography	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four polymorphs of IrI ( CO ) 2 ( OC ( CH3 ) CHC ( CH3 ) N ( p-tol ) ) have been characterized by single crystal X-ray crystallography .
	manualset3
231617	1	428075	15	NULL	NULL	0	NULL	Four polypeptides	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four polypeptides , the products of genes rIIA , rIIB , 39 , and 52 were operationally defined as membrane proteins .
	manualset3
231622	2	428075	15	NULL	NULL	0	NULL	 product of gene rIIA 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Four polypeptides , the products of genes rIIA , rIIB , 39 , and 52 were operationally defined as membrane proteins .
	manualset3
231624	3	428075	15	NULL	NULL	0	NULL	 product of gene rIIB	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Four polypeptides , the products of genes rIIA , rIIB , 39 , and 52 were operationally defined as membrane proteins .
	manualset3
231627	4	428075	15	NULL	NULL	0	NULL	 product of gene 39	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Four polypeptides , the products of genes rIIA , rIIB , 39 , and 52 were operationally defined as membrane proteins .
	manualset3
231628	5	428075	15	NULL	NULL	0	NULL	 product of gene 52	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Four polypeptides , the products of genes rIIA , rIIB , 39 , and 52 were operationally defined as membrane proteins .
	manualset3
231629	6	428075	15	NULL	NULL	NULL	NULL	membrane proteins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four polypeptides , the products of genes rIIA , rIIB , 39 , and 52 were operationally defined as membrane proteins .
	manualset3
231631	1	428076	15	NULL	NULL	0	NULL	Four small carcinomas	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four small carcinomas ( 3 , 6 , 10 , and 15 mm ) of the large intestine have been examined for residual epithelial polyp ; none was found .
	manualset3
231632	2	428076	15	NULL	NULL	0	NULL	3 mm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Four small carcinomas ( 3 , 6 , 10 , and 15 mm ) of the large intestine have been examined for residual epithelial polyp ; none was found .
	manualset3
231633	3	428076	15	NULL	NULL	0	NULL	6 mm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Four small carcinomas ( 3 , 6 , 10 , and 15 mm ) of the large intestine have been examined for residual epithelial polyp ; none was found .
	manualset3
231634	4	428076	15	NULL	NULL	0	NULL	10 mm	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Four small carcinomas ( 3 , 6 , 10 , and 15 mm ) of the large intestine have been examined for residual epithelial polyp ; none was found .
	manualset3
231635	5	428076	15	NULL	NULL	0	NULL	15 mm 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Four small carcinomas ( 3 , 6 , 10 , and 15 mm ) of the large intestine have been examined for residual epithelial polyp ; none was found .
	manualset3
231636	6	428076	15	NULL	NULL	0	NULL	large intestine	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Four small carcinomas ( 3 , 6 , 10 , and 15 mm ) of the large intestine have been examined for residual epithelial polyp ; none was found .
	manualset3
231637	7	428076	15	NULL	NULL	0	NULL	residual epithelial polyp	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Four small carcinomas ( 3 , 6 , 10 , and 15 mm ) of the large intestine have been examined for residual epithelial polyp ; none was found .
	manualset3
231641	1	428077	15	NULL	NULL	0	NULL	Resection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Resection of the large superficial petrosal nerve and post-otitic syndromes ) .
	manualset3
231642	2	428077	15	NULL	NULL	0	NULL	superficial petrosal nerve	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Resection of the large superficial petrosal nerve and post-otitic syndromes ) .
	manualset3
231643	3	428077	15	NULL	NULL	NULL	NULL	post-otitic syndromes	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Resection of the large superficial petrosal nerve and post-otitic syndromes ) .
	manualset3
231644	1	428078	15	NULL	NULL	NULL	NULL	Four species	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four species of rodents ( Apodemus agrarius , Apodemus peninsulae , Microtus fortis , and Clethrionomys rufocanus ) comprised 88.5 percent of 10 , 595 captured rodents and 94.1 percent of 996 antigen-positive animals .
	manualset3
231645	3	428078	15	NULL	NULL	NULL	NULL	Apodemus agrarius	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four species of rodents ( Apodemus agrarius , Apodemus peninsulae , Microtus fortis , and Clethrionomys rufocanus ) comprised 88.5 percent of 10 , 595 captured rodents and 94.1 percent of 996 antigen-positive animals .
	manualset3
231646	4	428078	15	NULL	NULL	NULL	NULL	Apodemus peninsulae	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four species of rodents ( Apodemus agrarius , Apodemus peninsulae , Microtus fortis , and Clethrionomys rufocanus ) comprised 88.5 percent of 10 , 595 captured rodents and 94.1 percent of 996 antigen-positive animals .
	manualset3
231647	5	428078	15	NULL	NULL	NULL	NULL	Microtus fortis	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four species of rodents ( Apodemus agrarius , Apodemus peninsulae , Microtus fortis , and Clethrionomys rufocanus ) comprised 88.5 percent of 10 , 595 captured rodents and 94.1 percent of 996 antigen-positive animals .
	manualset3
231648	6	428078	15	NULL	NULL	NULL	NULL	Clethrionomys rufocanus	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four species of rodents ( Apodemus agrarius , Apodemus peninsulae , Microtus fortis , and Clethrionomys rufocanus ) comprised 88.5 percent of 10 , 595 captured rodents and 94.1 percent of 996 antigen-positive animals .
	manualset3
231649	7	428078	15	NULL	NULL	NULL	NULL	88.5 percent 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four species of rodents ( Apodemus agrarius , Apodemus peninsulae , Microtus fortis , and Clethrionomys rufocanus ) comprised 88.5 percent of 10 , 595 captured rodents and 94.1 percent of 996 antigen-positive animals .
	manualset3
231650	8	428078	15	NULL	NULL	NULL	NULL	10 , 595 captured rodents	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four species of rodents ( Apodemus agrarius , Apodemus peninsulae , Microtus fortis , and Clethrionomys rufocanus ) comprised 88.5 percent of 10 , 595 captured rodents and 94.1 percent of 996 antigen-positive animals .
	manualset3
231651	9	428078	15	NULL	NULL	NULL	NULL	94.1 percent 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four species of rodents ( Apodemus agrarius , Apodemus peninsulae , Microtus fortis , and Clethrionomys rufocanus ) comprised 88.5 percent of 10 , 595 captured rodents and 94.1 percent of 996 antigen-positive animals .
	manualset3
231652	10	428078	15	NULL	NULL	NULL	NULL	996 antigen-positive animals	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four species of rodents ( Apodemus agrarius , Apodemus peninsulae , Microtus fortis , and Clethrionomys rufocanus ) comprised 88.5 percent of 10 , 595 captured rodents and 94.1 percent of 996 antigen-positive animals .
	manualset3
233044	2	428078	15	NULL	NULL	0	NULL	rodents	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Four species of rodents ( Apodemus agrarius , Apodemus peninsulae , Microtus fortis , and Clethrionomys rufocanus ) comprised 88.5 percent of 10 , 595 captured rodents and 94.1 percent of 996 antigen-positive animals .
	manualset3
231653	1	428079	15	NULL	NULL	0	NULL	Four strains	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four strains of lithotrophic sulfate-reducing bacteria ( SRB ) have been enriched and isolated from anoxic sediments of hypersaline chloride-sulfate lakes in the Kulunda Steppe ( Altai , Russia ) at 2M NaCl and pH 7.5 .
	manualset3
231654	2	428079	15	NULL	NULL	0	NULL	lithotrophic sulfate-reducing bacteria ( SRB )	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Four strains of lithotrophic sulfate-reducing bacteria ( SRB ) have been enriched and isolated from anoxic sediments of hypersaline chloride-sulfate lakes in the Kulunda Steppe ( Altai , Russia ) at 2M NaCl and pH 7.5 .
	manualset3
231655	3	428079	15	NULL	NULL	0	NULL	anoxic sediments	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Four strains of lithotrophic sulfate-reducing bacteria ( SRB ) have been enriched and isolated from anoxic sediments of hypersaline chloride-sulfate lakes in the Kulunda Steppe ( Altai , Russia ) at 2M NaCl and pH 7.5 .
	manualset3
231656	4	428079	15	NULL	NULL	0	NULL	hypersaline chloride-sulfate lakes	EnvironmentalFactor												NULL		0	NULL	NULL	NULL	NULL	NULL	Four strains of lithotrophic sulfate-reducing bacteria ( SRB ) have been enriched and isolated from anoxic sediments of hypersaline chloride-sulfate lakes in the Kulunda Steppe ( Altai , Russia ) at 2M NaCl and pH 7.5 .
	manualset3
231657	5	428079	15	NULL	NULL	NULL	NULL	Kulunda Steppe	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four strains of lithotrophic sulfate-reducing bacteria ( SRB ) have been enriched and isolated from anoxic sediments of hypersaline chloride-sulfate lakes in the Kulunda Steppe ( Altai , Russia ) at 2M NaCl and pH 7.5 .
	manualset3
231658	7	428079	15	NULL	NULL	NULL	NULL	2M NaCl	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four strains of lithotrophic sulfate-reducing bacteria ( SRB ) have been enriched and isolated from anoxic sediments of hypersaline chloride-sulfate lakes in the Kulunda Steppe ( Altai , Russia ) at 2M NaCl and pH 7.5 .
	manualset3
231659	8	428079	15	NULL	NULL	NULL	NULL	pH 7.5	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four strains of lithotrophic sulfate-reducing bacteria ( SRB ) have been enriched and isolated from anoxic sediments of hypersaline chloride-sulfate lakes in the Kulunda Steppe ( Altai , Russia ) at 2M NaCl and pH 7.5 .
	manualset3
233045	6	428079	15	NULL	NULL	0	NULL	Altai , Russia	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	Four strains of lithotrophic sulfate-reducing bacteria ( SRB ) have been enriched and isolated from anoxic sediments of hypersaline chloride-sulfate lakes in the Kulunda Steppe ( Altai , Russia ) at 2M NaCl and pH 7.5 .
	manualset3
231660	1	428080	15	NULL	NULL	0	NULL	Four strains	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Four strains of the Bacillus cereus group were compared for their germinant receptor composition and spore germination capacity .
	manualset3
231661	2	428080	15	NULL	NULL	0	NULL	Bacillus cereus group	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Four strains of the Bacillus cereus group were compared for their germinant receptor composition and spore germination capacity .
	manualset3
231662	3	428080	15	NULL	NULL	NULL	NULL	germinant receptor composition	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four strains of the Bacillus cereus group were compared for their germinant receptor composition and spore germination capacity .
	manualset3
231664	4	428080	15	NULL	NULL	0	NULL	spore germination capacity	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Four strains of the Bacillus cereus group were compared for their germinant receptor composition and spore germination capacity .
	manualset3
231671	1	428081	15	NULL	NULL	NULL	NULL	Four	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four subsequent studies focused on spatial-symbolic threat sensitivity and related it to right-wing authoritarianism , aversive reactions to unfamiliar out-groups , and revulsion to vermin .
	manualset3
231676	3	428081	15	NULL	NULL	NULL	NULL	spatial-symbolic threat sensitivity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four subsequent studies focused on spatial-symbolic threat sensitivity and related it to right-wing authoritarianism , aversive reactions to unfamiliar out-groups , and revulsion to vermin .
	manualset3
231677	4	428081	15	NULL	NULL	NULL	NULL	right-wing authoritarianism	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four subsequent studies focused on spatial-symbolic threat sensitivity and related it to right-wing authoritarianism , aversive reactions to unfamiliar out-groups , and revulsion to vermin .
	manualset3
231678	5	428081	15	NULL	NULL	NULL	NULL	aversive reactions	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four subsequent studies focused on spatial-symbolic threat sensitivity and related it to right-wing authoritarianism , aversive reactions to unfamiliar out-groups , and revulsion to vermin .
	manualset3
231679	8	428081	15	NULL	NULL	NULL	NULL	out-groups	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four subsequent studies focused on spatial-symbolic threat sensitivity and related it to right-wing authoritarianism , aversive reactions to unfamiliar out-groups , and revulsion to vermin .
	manualset3
231680	6	428081	15	NULL	NULL	0	NULL	revulsion	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Four subsequent studies focused on spatial-symbolic threat sensitivity and related it to right-wing authoritarianism , aversive reactions to unfamiliar out-groups , and revulsion to vermin .
	manualset3
231681	7	428081	15	NULL	NULL	0	NULL	vermin	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Four subsequent studies focused on spatial-symbolic threat sensitivity and related it to right-wing authoritarianism , aversive reactions to unfamiliar out-groups , and revulsion to vermin .
	manualset3
233046	2	428081	15	NULL	NULL	0	NULL	studies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Four subsequent studies focused on spatial-symbolic threat sensitivity and related it to right-wing authoritarianism , aversive reactions to unfamiliar out-groups , and revulsion to vermin .
	manualset3
231682	1	428082	15	NULL	NULL	NULL	NULL	Four transcription factors	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four transcription factors , COUP-TFI , Emx2 , Pax6 , and Sp8 , with graded expression across the embryonic cortical axes , are shown to determine sizes and positions of cortical areas by specifying or repressing area identities within cortical progenitors .
	manualset3
231684	3	428082	15	NULL	NULL	NULL	NULL	Emx2 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four transcription factors , COUP-TFI , Emx2 , Pax6 , and Sp8 , with graded expression across the embryonic cortical axes , are shown to determine sizes and positions of cortical areas by specifying or repressing area identities within cortical progenitors .
	manualset3
231685	4	428082	15	NULL	NULL	NULL	NULL	Pax6	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four transcription factors , COUP-TFI , Emx2 , Pax6 , and Sp8 , with graded expression across the embryonic cortical axes , are shown to determine sizes and positions of cortical areas by specifying or repressing area identities within cortical progenitors .
	manualset3
231686	5	428082	15	NULL	NULL	NULL	NULL	Sp8 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four transcription factors , COUP-TFI , Emx2 , Pax6 , and Sp8 , with graded expression across the embryonic cortical axes , are shown to determine sizes and positions of cortical areas by specifying or repressing area identities within cortical progenitors .
	manualset3
231687	6	428082	15	NULL	NULL	0	NULL	graded expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Four transcription factors , COUP-TFI , Emx2 , Pax6 , and Sp8 , with graded expression across the embryonic cortical axes , are shown to determine sizes and positions of cortical areas by specifying or repressing area identities within cortical progenitors .
	manualset3
231688	7	428082	15	NULL	NULL	0	NULL	embryonic cortical axes	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Four transcription factors , COUP-TFI , Emx2 , Pax6 , and Sp8 , with graded expression across the embryonic cortical axes , are shown to determine sizes and positions of cortical areas by specifying or repressing area identities within cortical progenitors .
	manualset3
231689	8	428082	15	NULL	NULL	NULL	NULL	sizes of cortical areas	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four transcription factors , COUP-TFI , Emx2 , Pax6 , and Sp8 , with graded expression across the embryonic cortical axes , are shown to determine sizes and positions of cortical areas by specifying or repressing area identities within cortical progenitors .
	manualset3
231690	10	428082	15	NULL	NULL	NULL	NULL	area identities	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four transcription factors , COUP-TFI , Emx2 , Pax6 , and Sp8 , with graded expression across the embryonic cortical axes , are shown to determine sizes and positions of cortical areas by specifying or repressing area identities within cortical progenitors .
	manualset3
231691	11	428082	15	NULL	NULL	NULL	NULL	cortical progenitors	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Four transcription factors , COUP-TFI , Emx2 , Pax6 , and Sp8 , with graded expression across the embryonic cortical axes , are shown to determine sizes and positions of cortical areas by specifying or repressing area identities within cortical progenitors .
	manualset3
233049	2	428082	15	NULL	NULL	0	NULL	 COUP-TFI	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Four transcription factors , COUP-TFI , Emx2 , Pax6 , and Sp8 , with graded expression across the embryonic cortical axes , are shown to determine sizes and positions of cortical areas by specifying or repressing area identities within cortical progenitors .
	manualset3
233054	9	428082	15	NULL	NULL	0	NULL	positions of cortical areas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Four transcription factors , COUP-TFI , Emx2 , Pax6 , and Sp8 , with graded expression across the embryonic cortical axes , are shown to determine sizes and positions of cortical areas by specifying or repressing area identities within cortical progenitors .
	manualset3
231683	1	428083	15	NULL	NULL	NULL	NULL	Fourier transformation infrared microspectroscopy ( FTIR-MSP ) mapping technique 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fourier transformation infrared microspectroscopy ( FTIR-MSP ) mapping technique can collect the infrared information from micro-samples and scan the tissue slides and cells .
	manualset3
231692	2	428083	15	NULL	NULL	NULL	NULL	infrared information	ExperimentalFactor												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fourier transformation infrared microspectroscopy ( FTIR-MSP ) mapping technique can collect the infrared information from micro-samples and scan the tissue slides and cells .
	manualset3
231693	3	428083	15	NULL	NULL	NULL	NULL	micro-samples	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fourier transformation infrared microspectroscopy ( FTIR-MSP ) mapping technique can collect the infrared information from micro-samples and scan the tissue slides and cells .
	manualset3
231694	4	428083	15	NULL	NULL	0	NULL	tissue slides	Tissue												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourier transformation infrared microspectroscopy ( FTIR-MSP ) mapping technique can collect the infrared information from micro-samples and scan the tissue slides and cells .
	manualset3
231695	5	428083	15	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourier transformation infrared microspectroscopy ( FTIR-MSP ) mapping technique can collect the infrared information from micro-samples and scan the tissue slides and cells .
	manualset3
231696	1	428084	15	NULL	NULL	NULL	NULL	Fourin vitrooxidant models	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fourin vitrooxidant and 2in vivoantiinflammation models were used to evaluate the pharmacological activities of the different pears .
	manualset3
231697	2	428084	15	NULL	NULL	NULL	NULL	2in vivoantiinflammation models	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fourin vitrooxidant and 2in vivoantiinflammation models were used to evaluate the pharmacological activities of the different pears .
	manualset3
231698	3	428084	15	NULL	NULL	0	NULL	pharmacological activities	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourin vitrooxidant and 2in vivoantiinflammation models were used to evaluate the pharmacological activities of the different pears .
	manualset3
231699	4	428084	15	NULL	NULL	0	NULL	pears	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourin vitrooxidant and 2in vivoantiinflammation models were used to evaluate the pharmacological activities of the different pears .
	manualset3
231700	1	428085	15	NULL	NULL	0	NULL	Fourteen month-old	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen - and 18-month-olds behaved systematically toward categories with different parts ( legs or wheels ) but not toward categories with matching parts ( legs or legs ) .
	manualset3
231701	2	428085	15	NULL	NULL	0	NULL	18-month-old	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen - and 18-month-olds behaved systematically toward categories with different parts ( legs or wheels ) but not toward categories with matching parts ( legs or legs ) .
	manualset3
231702	3	428085	15	NULL	NULL	NULL	NULL	categories	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fourteen - and 18-month-olds behaved systematically toward categories with different parts ( legs or wheels ) but not toward categories with matching parts ( legs or legs ) .
	manualset3
231703	7	428085	15	NULL	NULL	NULL	NULL	categories 	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fourteen - and 18-month-olds behaved systematically toward categories with different parts ( legs or wheels ) but not toward categories with matching parts ( legs or legs ) .
	manualset3
233055	4	428085	15	NULL	NULL	NULL	NULL	different parts 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fourteen - and 18-month-olds behaved systematically toward categories with different parts ( legs or wheels ) but not toward categories with matching parts ( legs or legs ) .
	manualset3
233056	5	428085	15	NULL	NULL	0	NULL	legs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen - and 18-month-olds behaved systematically toward categories with different parts ( legs or wheels ) but not toward categories with matching parts ( legs or legs ) .
	manualset3
233057	6	428085	15	NULL	NULL	0	NULL	wheels	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen - and 18-month-olds behaved systematically toward categories with different parts ( legs or wheels ) but not toward categories with matching parts ( legs or legs ) .
	manualset3
233058	8	428085	15	NULL	NULL	0	NULL	matching parts	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen - and 18-month-olds behaved systematically toward categories with different parts ( legs or wheels ) but not toward categories with matching parts ( legs or legs ) .
	manualset3
233059	9	428085	15	NULL	NULL	0	NULL	legs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen - and 18-month-olds behaved systematically toward categories with different parts ( legs or wheels ) but not toward categories with matching parts ( legs or legs ) .
	manualset3
233060	10	428085	15	NULL	NULL	0	NULL	legs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen - and 18-month-olds behaved systematically toward categories with different parts ( legs or wheels ) but not toward categories with matching parts ( legs or legs ) .
	manualset3
231704	1	428086	15	NULL	NULL	0	NULL	Resection	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Resection of the lungs in tuberculosis ) .
	manualset3
231705	2	428086	15	NULL	NULL	0	NULL	lungs	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Resection of the lungs in tuberculosis ) .
	manualset3
231706	3	428086	15	NULL	NULL	0	NULL	tuberculosis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Resection of the lungs in tuberculosis ) .
	manualset3
232017	1	428087	15	NULL	NULL	NULL	NULL	Fourteen GHD children	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fourteen GHD children were re-evaluated after 1 year of GH treatment : dermal thickness and skin stiffness were significantly improved ( p & lt ; 0.001 and p & lt ; 0.05 respectively ) while elasticity was not modified .
	manualset3
232018	2	428087	15	NULL	NULL	0	NULL	1 year	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen GHD children were re-evaluated after 1 year of GH treatment : dermal thickness and skin stiffness were significantly improved ( p & lt ; 0.001 and p & lt ; 0.05 respectively ) while elasticity was not modified .
	manualset3
232019	3	428087	15	NULL	NULL	0	NULL	GH treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen GHD children were re-evaluated after 1 year of GH treatment : dermal thickness and skin stiffness were significantly improved ( p & lt ; 0.001 and p & lt ; 0.05 respectively ) while elasticity was not modified .
	manualset3
232020	4	428087	15	NULL	NULL	0	NULL	dermal thickness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen GHD children were re-evaluated after 1 year of GH treatment : dermal thickness and skin stiffness were significantly improved ( p & lt ; 0.001 and p & lt ; 0.05 respectively ) while elasticity was not modified .
	manualset3
232021	5	428087	15	NULL	NULL	0	NULL	skin stiffness	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen GHD children were re-evaluated after 1 year of GH treatment : dermal thickness and skin stiffness were significantly improved ( p & lt ; 0.001 and p & lt ; 0.05 respectively ) while elasticity was not modified .
	manualset3
232022	6	428087	15	NULL	NULL	0	NULL	p & lt ; 0.001	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen GHD children were re-evaluated after 1 year of GH treatment : dermal thickness and skin stiffness were significantly improved ( p & lt ; 0.001 and p & lt ; 0.05 respectively ) while elasticity was not modified .
	manualset3
232023	7	428087	15	NULL	NULL	0	NULL	 p & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen GHD children were re-evaluated after 1 year of GH treatment : dermal thickness and skin stiffness were significantly improved ( p & lt ; 0.001 and p & lt ; 0.05 respectively ) while elasticity was not modified .
	manualset3
232024	8	428087	15	NULL	NULL	0	NULL	elasticity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen GHD children were re-evaluated after 1 year of GH treatment : dermal thickness and skin stiffness were significantly improved ( p & lt ; 0.001 and p & lt ; 0.05 respectively ) while elasticity was not modified .
	manualset3
232025	1	428088	15	NULL	NULL	0	NULL	Fourteen months later	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen months later a recurrence of the MALT lymphoma involving both sides of the diaphragm was found and was treated with chemoimmunotherapy .
	manualset3
232026	2	428088	15	NULL	NULL	0	NULL	recurrence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen months later a recurrence of the MALT lymphoma involving both sides of the diaphragm was found and was treated with chemoimmunotherapy .
	manualset3
232027	3	428088	15	NULL	NULL	0	NULL	MALT lymphoma	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen months later a recurrence of the MALT lymphoma involving both sides of the diaphragm was found and was treated with chemoimmunotherapy .
	manualset3
232028	4	428088	15	NULL	NULL	0	NULL	both sides of the diaphragm	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen months later a recurrence of the MALT lymphoma involving both sides of the diaphragm was found and was treated with chemoimmunotherapy .
	manualset3
232029	5	428088	15	NULL	NULL	0	NULL	chemoimmunotherapy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen months later a recurrence of the MALT lymphoma involving both sides of the diaphragm was found and was treated with chemoimmunotherapy .
	manualset3
232030	1	428089	15	NULL	NULL	0	NULL	Fourteen	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen of those GOI also presented differences in expression ( p & lt ; 0.05 ) following exposure to the threshold concentration of bacterial TBP-containing extract .
	manualset3
232031	2	428089	15	NULL	NULL	0	NULL	GOI	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen of those GOI also presented differences in expression ( p & lt ; 0.05 ) following exposure to the threshold concentration of bacterial TBP-containing extract .
	manualset3
232032	3	428089	15	NULL	NULL	0	NULL	differences	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen of those GOI also presented differences in expression ( p & lt ; 0.05 ) following exposure to the threshold concentration of bacterial TBP-containing extract .
	manualset3
232033	4	428089	15	NULL	NULL	0	NULL	expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen of those GOI also presented differences in expression ( p & lt ; 0.05 ) following exposure to the threshold concentration of bacterial TBP-containing extract .
	manualset3
232034	5	428089	15	NULL	NULL	0	NULL	p & lt ; 0.05 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen of those GOI also presented differences in expression ( p & lt ; 0.05 ) following exposure to the threshold concentration of bacterial TBP-containing extract .
	manualset3
232035	6	428089	15	NULL	NULL	0	NULL	exposure 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen of those GOI also presented differences in expression ( p & lt ; 0.05 ) following exposure to the threshold concentration of bacterial TBP-containing extract .
	manualset3
232036	7	428089	15	NULL	NULL	0	NULL	threshold concentration 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen of those GOI also presented differences in expression ( p & lt ; 0.05 ) following exposure to the threshold concentration of bacterial TBP-containing extract .
	manualset3
232037	8	428089	15	NULL	NULL	NULL	NULL	bacterial TBP-containing extract 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fourteen of those GOI also presented differences in expression ( p & lt ; 0.05 ) following exposure to the threshold concentration of bacterial TBP-containing extract .
	manualset3
232039	1	428090	15	NULL	NULL	NULL	NULL	Fourteen patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fourteen patients with histologically confirmed prostate cancer and five patients with benign prostatic hyperplasia were studied with ( ( 11 ) C ) choline PET .
	manualset3
232040	2	428090	15	NULL	NULL	0	NULL	prostate cancer	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen patients with histologically confirmed prostate cancer and five patients with benign prostatic hyperplasia were studied with ( ( 11 ) C ) choline PET .
	manualset3
232041	3	428090	15	NULL	NULL	NULL	NULL	five patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fourteen patients with histologically confirmed prostate cancer and five patients with benign prostatic hyperplasia were studied with ( ( 11 ) C ) choline PET .
	manualset3
232042	4	428090	15	NULL	NULL	0	NULL	benign prostatic hyperplasia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen patients with histologically confirmed prostate cancer and five patients with benign prostatic hyperplasia were studied with ( ( 11 ) C ) choline PET .
	manualset3
232043	5	428090	15	NULL	NULL	0	NULL	( ( 11 ) C ) choline PET	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen patients with histologically confirmed prostate cancer and five patients with benign prostatic hyperplasia were studied with ( ( 11 ) C ) choline PET .
	manualset3
232052	1	428091	15	NULL	NULL	NULL	NULL	Fourteen patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fourteen patients with renovascular hypertension complicated by renal impairment and/or a nonfunctioning kidney underwent percutaneous transluminal angioplasty of the remaining kidney ( s ) for the purpose of improving blood pressure control and/or renal function .
	manualset3
232053	2	428091	15	NULL	NULL	0	NULL	renovascular hypertension	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen patients with renovascular hypertension complicated by renal impairment and/or a nonfunctioning kidney underwent percutaneous transluminal angioplasty of the remaining kidney ( s ) for the purpose of improving blood pressure control and/or renal function .
	manualset3
232054	3	428091	15	NULL	NULL	0	NULL	renal impairment	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen patients with renovascular hypertension complicated by renal impairment and/or a nonfunctioning kidney underwent percutaneous transluminal angioplasty of the remaining kidney ( s ) for the purpose of improving blood pressure control and/or renal function .
	manualset3
232055	4	428091	15	NULL	NULL	0	NULL	kidney	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen patients with renovascular hypertension complicated by renal impairment and/or a nonfunctioning kidney underwent percutaneous transluminal angioplasty of the remaining kidney ( s ) for the purpose of improving blood pressure control and/or renal function .
	manualset3
232056	5	428091	15	NULL	NULL	0	NULL	percutaneous transluminal angioplasty 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen patients with renovascular hypertension complicated by renal impairment and/or a nonfunctioning kidney underwent percutaneous transluminal angioplasty of the remaining kidney ( s ) for the purpose of improving blood pressure control and/or renal function .
	manualset3
232057	6	428091	15	NULL	NULL	0	NULL	kidney ( s ) 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen patients with renovascular hypertension complicated by renal impairment and/or a nonfunctioning kidney underwent percutaneous transluminal angioplasty of the remaining kidney ( s ) for the purpose of improving blood pressure control and/or renal function .
	manualset3
232058	7	428091	15	NULL	NULL	0	NULL	purpose	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen patients with renovascular hypertension complicated by renal impairment and/or a nonfunctioning kidney underwent percutaneous transluminal angioplasty of the remaining kidney ( s ) for the purpose of improving blood pressure control and/or renal function .
	manualset3
232059	8	428091	15	NULL	NULL	NULL	NULL	blood pressure control	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fourteen patients with renovascular hypertension complicated by renal impairment and/or a nonfunctioning kidney underwent percutaneous transluminal angioplasty of the remaining kidney ( s ) for the purpose of improving blood pressure control and/or renal function .
	manualset3
232060	9	428091	15	NULL	NULL	0	NULL	renal function 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen patients with renovascular hypertension complicated by renal impairment and/or a nonfunctioning kidney underwent percutaneous transluminal angioplasty of the remaining kidney ( s ) for the purpose of improving blood pressure control and/or renal function .
	manualset3
232061	1	428092	15	NULL	NULL	NULL	NULL	Fourteen untreated patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fourteen untreated patients with non-insulin-dependent diabetes mellitus ( NIDDM ) and 15 healthy control subjects were studied .
	manualset3
232062	2	428092	15	NULL	NULL	0	NULL	non-insulin-dependent diabetes mellitus ( NIDDM )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen untreated patients with non-insulin-dependent diabetes mellitus ( NIDDM ) and 15 healthy control subjects were studied .
	manualset3
232063	3	428092	15	NULL	NULL	NULL	NULL	15 healthy control subjects 	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fourteen untreated patients with non-insulin-dependent diabetes mellitus ( NIDDM ) and 15 healthy control subjects were studied .
	manualset3
232064	1	428093	15	NULL	NULL	NULL	NULL	Addiction	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Addiction to cocaine : A risk factor for suicide ? ) .
	manualset3
232065	2	428093	15	NULL	NULL	NULL	NULL	cocaine	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Addiction to cocaine : A risk factor for suicide ? ) .
	manualset3
232066	3	428093	15	NULL	NULL	NULL	NULL	risk factor	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Addiction to cocaine : A risk factor for suicide ? ) .
	manualset3
232067	4	428093	15	NULL	NULL	0	NULL	suicide	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Addiction to cocaine : A risk factor for suicide ? ) .
	manualset3
232068	1	428094	15	NULL	NULL	0	NULL	Respiratory function 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Respiratory function after open heart surgery ( author 's transl ) ) .
	manualset3
232069	2	428094	15	NULL	NULL	0	NULL	open heart surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Respiratory function after open heart surgery ( author 's transl ) ) .
	manualset3
232070	3	428094	15	NULL	NULL	0	NULL	 author 's transl	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Respiratory function after open heart surgery ( author 's transl ) ) .
	manualset3
232071	1	428095	15	NULL	NULL	0	NULL	Fourteen 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen were evaluated before laparotomy ( group I ) , 25 following surgical treatment ( group II ) , and 8 were followed by CT in the course , or following chemotherapy with or without radiation therapy ( group III ) .
	manualset3
232072	2	428095	15	NULL	NULL	0	NULL	laparotomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen were evaluated before laparotomy ( group I ) , 25 following surgical treatment ( group II ) , and 8 were followed by CT in the course , or following chemotherapy with or without radiation therapy ( group III ) .
	manualset3
232073	3	428095	15	NULL	NULL	0	NULL	group I	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen were evaluated before laparotomy ( group I ) , 25 following surgical treatment ( group II ) , and 8 were followed by CT in the course , or following chemotherapy with or without radiation therapy ( group III ) .
	manualset3
232074	4	428095	15	NULL	NULL	0	NULL	25	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen were evaluated before laparotomy ( group I ) , 25 following surgical treatment ( group II ) , and 8 were followed by CT in the course , or following chemotherapy with or without radiation therapy ( group III ) .
	manualset3
232075	5	428095	15	NULL	NULL	0	NULL	surgical treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen were evaluated before laparotomy ( group I ) , 25 following surgical treatment ( group II ) , and 8 were followed by CT in the course , or following chemotherapy with or without radiation therapy ( group III ) .
	manualset3
232076	6	428095	15	NULL	NULL	0	NULL	group II	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen were evaluated before laparotomy ( group I ) , 25 following surgical treatment ( group II ) , and 8 were followed by CT in the course , or following chemotherapy with or without radiation therapy ( group III ) .
	manualset3
232077	7	428095	15	NULL	NULL	0	NULL	 8 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen were evaluated before laparotomy ( group I ) , 25 following surgical treatment ( group II ) , and 8 were followed by CT in the course , or following chemotherapy with or without radiation therapy ( group III ) .
	manualset3
232078	8	428095	15	NULL	NULL	0	NULL	CT	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen were evaluated before laparotomy ( group I ) , 25 following surgical treatment ( group II ) , and 8 were followed by CT in the course , or following chemotherapy with or without radiation therapy ( group III ) .
	manualset3
232079	9	428095	15	NULL	NULL	0	NULL	course	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen were evaluated before laparotomy ( group I ) , 25 following surgical treatment ( group II ) , and 8 were followed by CT in the course , or following chemotherapy with or without radiation therapy ( group III ) .
	manualset3
232080	10	428095	15	NULL	NULL	0	NULL	chemotherapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen were evaluated before laparotomy ( group I ) , 25 following surgical treatment ( group II ) , and 8 were followed by CT in the course , or following chemotherapy with or without radiation therapy ( group III ) .
	manualset3
232081	11	428095	15	NULL	NULL	0	NULL	radiation therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen were evaluated before laparotomy ( group I ) , 25 following surgical treatment ( group II ) , and 8 were followed by CT in the course , or following chemotherapy with or without radiation therapy ( group III ) .
	manualset3
232084	12	428095	15	NULL	NULL	0	NULL	group III	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourteen were evaluated before laparotomy ( group I ) , 25 following surgical treatment ( group II ) , and 8 were followed by CT in the course , or following chemotherapy with or without radiation therapy ( group III ) .
	manualset3
232092	1	428096	15	NULL	NULL	0	NULL	Fourth	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourth , each area of cerebral cortex contributing to eye movements is discussed .
	manualset3
232093	2	428096	15	NULL	NULL	0	NULL	area of cerebral cortex	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourth , each area of cerebral cortex contributing to eye movements is discussed .
	manualset3
232094	3	428096	15	NULL	NULL	0	NULL	eye movements	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fourth , each area of cerebral cortex contributing to eye movements is discussed .
	manualset3
232100	1	428097	15	NULL	NULL	0	NULL	Fraction III	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Fraction III contains lactic acid as the effective principle ; the compositions of the other two have not been clarified yet .
	manualset3
232101	2	428097	15	NULL	NULL	0	NULL	lactic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Fraction III contains lactic acid as the effective principle ; the compositions of the other two have not been clarified yet .
	manualset3
232102	3	428097	15	NULL	NULL	NULL	NULL	effective principle	NamedEntity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fraction III contains lactic acid as the effective principle ; the compositions of the other two have not been clarified yet .
	manualset3
232125	4	428097	15	NULL	NULL	0	NULL	compositions	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Fraction III contains lactic acid as the effective principle ; the compositions of the other two have not been clarified yet .
	manualset3
232128	5	428097	15	NULL	NULL	0	NULL	two	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Fraction III contains lactic acid as the effective principle ; the compositions of the other two have not been clarified yet .
	manualset3
232103	1	428098	15	NULL	NULL	NULL	NULL	Fractional catabolic rate 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fractional catabolic rate of apoA-I was found to be significantly increased by 59 % to 0.360 + / - 0.084 / d in ESRD-HD patients as compared with control subjects of 0.227 + / - 0.076 / d ( P = 0.028 ) , whereas the production rates remained unchanged .
	manualset3
232104	2	428098	15	NULL	NULL	0	NULL	apoA-I 	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractional catabolic rate of apoA-I was found to be significantly increased by 59 % to 0.360 + / - 0.084 / d in ESRD-HD patients as compared with control subjects of 0.227 + / - 0.076 / d ( P = 0.028 ) , whereas the production rates remained unchanged .
	manualset3
232105	3	428098	15	NULL	NULL	0	NULL	59 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractional catabolic rate of apoA-I was found to be significantly increased by 59 % to 0.360 + / - 0.084 / d in ESRD-HD patients as compared with control subjects of 0.227 + / - 0.076 / d ( P = 0.028 ) , whereas the production rates remained unchanged .
	manualset3
232106	4	428098	15	NULL	NULL	0	NULL	0.360 + / - 0.084 / d 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractional catabolic rate of apoA-I was found to be significantly increased by 59 % to 0.360 + / - 0.084 / d in ESRD-HD patients as compared with control subjects of 0.227 + / - 0.076 / d ( P = 0.028 ) , whereas the production rates remained unchanged .
	manualset3
232107	5	428098	15	NULL	NULL	0	NULL	ESRD-HD patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractional catabolic rate of apoA-I was found to be significantly increased by 59 % to 0.360 + / - 0.084 / d in ESRD-HD patients as compared with control subjects of 0.227 + / - 0.076 / d ( P = 0.028 ) , whereas the production rates remained unchanged .
	manualset3
232108	6	428098	15	NULL	NULL	0	NULL	control subjects	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractional catabolic rate of apoA-I was found to be significantly increased by 59 % to 0.360 + / - 0.084 / d in ESRD-HD patients as compared with control subjects of 0.227 + / - 0.076 / d ( P = 0.028 ) , whereas the production rates remained unchanged .
	manualset3
232109	7	428098	15	NULL	NULL	0	NULL	0.227 + / - 0.076 / d	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractional catabolic rate of apoA-I was found to be significantly increased by 59 % to 0.360 + / - 0.084 / d in ESRD-HD patients as compared with control subjects of 0.227 + / - 0.076 / d ( P = 0.028 ) , whereas the production rates remained unchanged .
	manualset3
232110	8	428098	15	NULL	NULL	0	NULL	P = 0.028 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractional catabolic rate of apoA-I was found to be significantly increased by 59 % to 0.360 + / - 0.084 / d in ESRD-HD patients as compared with control subjects of 0.227 + / - 0.076 / d ( P = 0.028 ) , whereas the production rates remained unchanged .
	manualset3
232111	9	428098	15	NULL	NULL	0	NULL	production rates	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractional catabolic rate of apoA-I was found to be significantly increased by 59 % to 0.360 + / - 0.084 / d in ESRD-HD patients as compared with control subjects of 0.227 + / - 0.076 / d ( P = 0.028 ) , whereas the production rates remained unchanged .
	manualset3
232112	1	428099	15	NULL	NULL	0	NULL	Fractional composition	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractional composition of blood serum lipoproteins in mice and rats with Triton WR 1339-induced lipemia .
	manualset3
232113	2	428099	15	NULL	NULL	NULL	NULL	blood serum lipoproteins	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fractional composition of blood serum lipoproteins in mice and rats with Triton WR 1339-induced lipemia .
	manualset3
232114	3	428099	15	NULL	NULL	0	NULL	 mice	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractional composition of blood serum lipoproteins in mice and rats with Triton WR 1339-induced lipemia .
	manualset3
232115	4	428099	15	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractional composition of blood serum lipoproteins in mice and rats with Triton WR 1339-induced lipemia .
	manualset3
232116	5	428099	15	NULL	NULL	0	NULL	Triton WR 1339	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractional composition of blood serum lipoproteins in mice and rats with Triton WR 1339-induced lipemia .
	manualset3
232117	6	428099	15	NULL	NULL	0	NULL	lipemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractional composition of blood serum lipoproteins in mice and rats with Triton WR 1339-induced lipemia .
	manualset3
232118	1	428100	15	NULL	NULL	NULL	NULL	Fractional reserve	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fractional reserve of blood flow conception ) .
	manualset3
232119	2	428100	15	NULL	NULL	NULL	NULL	blood flow	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fractional reserve of blood flow conception ) .
	manualset3
232120	3	428100	15	NULL	NULL	0	NULL	conception 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractional reserve of blood flow conception ) .
	manualset3
232747	1	428101	15	NULL	NULL	0	NULL	Fractional volumes	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractional volumes of lysosomal-vacuolar elements and long lived protein degradation were quantitatively correlated in rat livers perfused in the single pass mode with varying levels of plasma amino acids .
	manualset3
232748	2	428101	15	NULL	NULL	0	NULL	lysosomal-vacuolar elements	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractional volumes of lysosomal-vacuolar elements and long lived protein degradation were quantitatively correlated in rat livers perfused in the single pass mode with varying levels of plasma amino acids .
	manualset3
232749	3	428101	15	NULL	NULL	0	NULL	protein degradation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractional volumes of lysosomal-vacuolar elements and long lived protein degradation were quantitatively correlated in rat livers perfused in the single pass mode with varying levels of plasma amino acids .
	manualset3
232750	4	428101	15	NULL	NULL	0	NULL	rat livers	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractional volumes of lysosomal-vacuolar elements and long lived protein degradation were quantitatively correlated in rat livers perfused in the single pass mode with varying levels of plasma amino acids .
	manualset3
232751	5	428101	15	NULL	NULL	NULL	NULL	single pass mode	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fractional volumes of lysosomal-vacuolar elements and long lived protein degradation were quantitatively correlated in rat livers perfused in the single pass mode with varying levels of plasma amino acids .
	manualset3
232752	6	428101	15	NULL	NULL	0	NULL	levels 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractional volumes of lysosomal-vacuolar elements and long lived protein degradation were quantitatively correlated in rat livers perfused in the single pass mode with varying levels of plasma amino acids .
	manualset3
232753	7	428101	15	NULL	NULL	0	NULL	 plasma amino acids	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractional volumes of lysosomal-vacuolar elements and long lived protein degradation were quantitatively correlated in rat livers perfused in the single pass mode with varying levels of plasma amino acids .
	manualset3
232754	1	428102	15	NULL	NULL	NULL	NULL	Fractionation	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fractionation of the complementary strands of coliphage lambda DNA based on the asymmetric distribution of the poly I , G-binding sites .
	manualset3
232755	2	428102	15	NULL	NULL	0	NULL	complementary strands	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractionation of the complementary strands of coliphage lambda DNA based on the asymmetric distribution of the poly I , G-binding sites .
	manualset3
232756	3	428102	15	NULL	NULL	0	NULL	coliphage lambda DNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractionation of the complementary strands of coliphage lambda DNA based on the asymmetric distribution of the poly I , G-binding sites .
	manualset3
232757	4	428102	15	NULL	NULL	0	NULL	asymmetric distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractionation of the complementary strands of coliphage lambda DNA based on the asymmetric distribution of the poly I , G-binding sites .
	manualset3
232758	5	428102	15	NULL	NULL	0	NULL	poly I binding sites	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractionation of the complementary strands of coliphage lambda DNA based on the asymmetric distribution of the poly I , G-binding sites .
	manualset3
232759	6	428102	15	NULL	NULL	0	NULL	Poly G-binding sites	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractionation of the complementary strands of coliphage lambda DNA based on the asymmetric distribution of the poly I , G-binding sites .
	manualset3
232760	1	428103	15	NULL	NULL	NULL	NULL	Fractionation	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fractionation of the native glycoprotein from the cat by gel chromatography in the presence of urea and dithiothreitol suggests a value of about 3 X 10 ( 6 ) for the molecular weights .
	manualset3
232761	2	428103	15	NULL	NULL	0	NULL	native glycoprotein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractionation of the native glycoprotein from the cat by gel chromatography in the presence of urea and dithiothreitol suggests a value of about 3 X 10 ( 6 ) for the molecular weights .
	manualset3
232762	3	428103	15	NULL	NULL	0	NULL	cat 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractionation of the native glycoprotein from the cat by gel chromatography in the presence of urea and dithiothreitol suggests a value of about 3 X 10 ( 6 ) for the molecular weights .
	manualset3
232763	4	428103	15	NULL	NULL	NULL	NULL	gel chromatography	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fractionation of the native glycoprotein from the cat by gel chromatography in the presence of urea and dithiothreitol suggests a value of about 3 X 10 ( 6 ) for the molecular weights .
	manualset3
232764	5	428103	15	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractionation of the native glycoprotein from the cat by gel chromatography in the presence of urea and dithiothreitol suggests a value of about 3 X 10 ( 6 ) for the molecular weights .
	manualset3
232765	6	428103	15	NULL	NULL	0	NULL	urea	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractionation of the native glycoprotein from the cat by gel chromatography in the presence of urea and dithiothreitol suggests a value of about 3 X 10 ( 6 ) for the molecular weights .
	manualset3
232766	7	428103	15	NULL	NULL	0	NULL	dithiothreitol	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractionation of the native glycoprotein from the cat by gel chromatography in the presence of urea and dithiothreitol suggests a value of about 3 X 10 ( 6 ) for the molecular weights .
	manualset3
232767	8	428103	15	NULL	NULL	NULL	NULL	value of about 3 X 10 ( 6 ) 	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fractionation of the native glycoprotein from the cat by gel chromatography in the presence of urea and dithiothreitol suggests a value of about 3 X 10 ( 6 ) for the molecular weights .
	manualset3
232768	9	428103	15	NULL	NULL	0	NULL	molecular weights	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Fractionation of the native glycoprotein from the cat by gel chromatography in the presence of urea and dithiothreitol suggests a value of about 3 X 10 ( 6 ) for the molecular weights .
	manualset3
232769	1	428104	15	NULL	NULL	0	NULL	Fracture behavior	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Fracture behavior of polypropylene/clay nanocomposites .
	manualset3
232770	2	428104	15	NULL	NULL	0	NULL	polypropylene nanocomposites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Fracture behavior of polypropylene/clay nanocomposites .
	manualset3
232771	3	428104	15	NULL	NULL	0	NULL	clay nanocomposites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Fracture behavior of polypropylene/clay nanocomposites .
	manualset3
232772	1	428105	15	NULL	NULL	0	NULL	Fragment Th26	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	Fragment Th26 is composed of amino acids Phe63-His291 .
	manualset3
232773	2	428105	15	NULL	NULL	NULL	NULL	amino acids Phe63-His291	PartOfProtein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fragment Th26 is composed of amino acids Phe63-His291 .
	manualset3
232774	1	428106	15	NULL	NULL	0	NULL	Fragmentation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fragmentation of fibronectin by inherent autolytic and matrix metalloproteinase activities .
	manualset3
232775	2	428106	15	NULL	NULL	0	NULL	fibronectin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Fragmentation of fibronectin by inherent autolytic and matrix metalloproteinase activities .
	manualset3
232776	3	428106	15	NULL	NULL	0	NULL	inherent autolytic activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fragmentation of fibronectin by inherent autolytic and matrix metalloproteinase activities .
	manualset3
232777	4	428106	15	NULL	NULL	0	NULL	matrix metalloproteinase activities	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fragmentation of fibronectin by inherent autolytic and matrix metalloproteinase activities .
	manualset3
232778	1	428107	15	NULL	NULL	NULL	NULL	Fragments	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fragments from seven loci in 107 kb of DNA migrated anomalously slow and these fragments contained blocks of A2-6 in a 10-11 base periodicity which is indicative of bent DNA .
	manualset3
232779	2	428107	15	NULL	NULL	0	NULL	seven loci	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Fragments from seven loci in 107 kb of DNA migrated anomalously slow and these fragments contained blocks of A2-6 in a 10-11 base periodicity which is indicative of bent DNA .
	manualset3
232780	3	428107	15	NULL	NULL	NULL	NULL	107 kb of DNA	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fragments from seven loci in 107 kb of DNA migrated anomalously slow and these fragments contained blocks of A2-6 in a 10-11 base periodicity which is indicative of bent DNA .
	manualset3
232781	4	428107	15	NULL	NULL	NULL	NULL	fragments	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fragments from seven loci in 107 kb of DNA migrated anomalously slow and these fragments contained blocks of A2-6 in a 10-11 base periodicity which is indicative of bent DNA .
	manualset3
232782	5	428107	15	NULL	NULL	0	NULL	blocks of A2-6 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Fragments from seven loci in 107 kb of DNA migrated anomalously slow and these fragments contained blocks of A2-6 in a 10-11 base periodicity which is indicative of bent DNA .
	manualset3
232783	6	428107	15	NULL	NULL	0	NULL	10-11 base periodicity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Fragments from seven loci in 107 kb of DNA migrated anomalously slow and these fragments contained blocks of A2-6 in a 10-11 base periodicity which is indicative of bent DNA .
	manualset3
232784	7	428107	15	NULL	NULL	NULL	NULL	DNA 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fragments from seven loci in 107 kb of DNA migrated anomalously slow and these fragments contained blocks of A2-6 in a 10-11 base periodicity which is indicative of bent DNA .
	manualset3
232812	1	428108	15	NULL	NULL	0	NULL	Frames of reference	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Frames of reference are coordinate systems used to compute and specify the location of objects with respect to other objects .
	manualset3
232813	2	428108	15	NULL	NULL	0	NULL	coordinate systems	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Frames of reference are coordinate systems used to compute and specify the location of objects with respect to other objects .
	manualset3
232814	3	428108	15	NULL	NULL	0	NULL	compute 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Frames of reference are coordinate systems used to compute and specify the location of objects with respect to other objects .
	manualset3
232815	4	428108	15	NULL	NULL	0	NULL	location	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Frames of reference are coordinate systems used to compute and specify the location of objects with respect to other objects .
	manualset3
232816	5	428108	15	NULL	NULL	0	NULL	objects	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Frames of reference are coordinate systems used to compute and specify the location of objects with respect to other objects .
	manualset3
232817	6	428108	15	NULL	NULL	0	NULL	objects	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Frames of reference are coordinate systems used to compute and specify the location of objects with respect to other objects .
	manualset3
232785	1	428109	15	NULL	NULL	0	NULL	Fraud	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fraud and misconduct in medical research .
	manualset3
232786	2	428109	15	NULL	NULL	0	NULL	misconduct	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fraud and misconduct in medical research .
	manualset3
232787	3	428109	15	NULL	NULL	0	NULL	medical research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Fraud and misconduct in medical research .
	manualset3
232788	1	428110	15	NULL	NULL	0	NULL	cyanobacteria	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Free-living cyanobacteria produce 0.3 microg/g BMAA , but produce 2-37 microg/g as symbionts in the coralloid roots of cycad trees .
	manualset3
232789	2	428110	15	NULL	NULL	0	NULL	0.3 microg/g	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Free-living cyanobacteria produce 0.3 microg/g BMAA , but produce 2-37 microg/g as symbionts in the coralloid roots of cycad trees .
	manualset3
232790	3	428110	15	NULL	NULL	0	NULL	BMAA	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Free-living cyanobacteria produce 0.3 microg/g BMAA , but produce 2-37 microg/g as symbionts in the coralloid roots of cycad trees .
	manualset3
232791	4	428110	15	NULL	NULL	0	NULL	2-37 microg/g	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Free-living cyanobacteria produce 0.3 microg/g BMAA , but produce 2-37 microg/g as symbionts in the coralloid roots of cycad trees .
	manualset3
232792	5	428110	15	NULL	NULL	0	NULL	symbionts 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Free-living cyanobacteria produce 0.3 microg/g BMAA , but produce 2-37 microg/g as symbionts in the coralloid roots of cycad trees .
	manualset3
232793	6	428110	15	NULL	NULL	0	NULL	coralloid roots	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Free-living cyanobacteria produce 0.3 microg/g BMAA , but produce 2-37 microg/g as symbionts in the coralloid roots of cycad trees .
	manualset3
232794	7	428110	15	NULL	NULL	0	NULL	cycad trees	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Free-living cyanobacteria produce 0.3 microg/g BMAA , but produce 2-37 microg/g as symbionts in the coralloid roots of cycad trees .
	manualset3
232795	1	428111	15	NULL	NULL	NULL	NULL	Free-operant performance	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Free-operant performance is also distinguished from discrete-trial performance .
	manualset3
232796	2	428111	15	NULL	NULL	NULL	NULL	discrete-trial performance	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Free-operant performance is also distinguished from discrete-trial performance .
	manualset3
232797	1	428112	15	NULL	NULL	NULL	NULL	chondroitin sulphate chains	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Free chondroitin sulphate chains initiated by galactoside were isolated and degraded to yield 3-O-beta-D-glucuronosyl D-galactose ( GlcA-Gal ) derived from the sequence , GlcA-Gal-Gal-Xyl-Ser , which links the polysaccharide to protein .
	manualset3
232798	2	428112	15	NULL	NULL	NULL	NULL	galactoside	NonProteinOrNucleicAcidChemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Free chondroitin sulphate chains initiated by galactoside were isolated and degraded to yield 3-O-beta-D-glucuronosyl D-galactose ( GlcA-Gal ) derived from the sequence , GlcA-Gal-Gal-Xyl-Ser , which links the polysaccharide to protein .
	manualset3
232799	3	428112	15	NULL	NULL	0	NULL	3-O-beta-D-glucuronosyl D-galactose ( GlcA-Gal ) 	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Free chondroitin sulphate chains initiated by galactoside were isolated and degraded to yield 3-O-beta-D-glucuronosyl D-galactose ( GlcA-Gal ) derived from the sequence , GlcA-Gal-Gal-Xyl-Ser , which links the polysaccharide to protein .
	manualset3
232800	4	428112	15	NULL	NULL	0	NULL	sequence	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Free chondroitin sulphate chains initiated by galactoside were isolated and degraded to yield 3-O-beta-D-glucuronosyl D-galactose ( GlcA-Gal ) derived from the sequence , GlcA-Gal-Gal-Xyl-Ser , which links the polysaccharide to protein .
	manualset3
232801	5	428112	15	NULL	NULL	0	NULL	GlcA-Gal-Gal-Xyl-Ser	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Free chondroitin sulphate chains initiated by galactoside were isolated and degraded to yield 3-O-beta-D-glucuronosyl D-galactose ( GlcA-Gal ) derived from the sequence , GlcA-Gal-Gal-Xyl-Ser , which links the polysaccharide to protein .
	manualset3
232802	6	428112	15	NULL	NULL	0	NULL	polysaccharide	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Free chondroitin sulphate chains initiated by galactoside were isolated and degraded to yield 3-O-beta-D-glucuronosyl D-galactose ( GlcA-Gal ) derived from the sequence , GlcA-Gal-Gal-Xyl-Ser , which links the polysaccharide to protein .
	manualset3
232803	7	428112	15	NULL	NULL	0	NULL	protein 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Free chondroitin sulphate chains initiated by galactoside were isolated and degraded to yield 3-O-beta-D-glucuronosyl D-galactose ( GlcA-Gal ) derived from the sequence , GlcA-Gal-Gal-Xyl-Ser , which links the polysaccharide to protein .
	manualset3
232804	1	428113	15	NULL	NULL	0	NULL	Free fatty acid ( FFA )	NonProteinOrNucleicAcidChemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Free fatty acid ( FFA ) metabolism was studied in 18 traumatized and/or septic patients .
	manualset3
232805	2	428113	15	NULL	NULL	NULL	NULL	metabolism	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Free fatty acid ( FFA ) metabolism was studied in 18 traumatized and/or septic patients .
	manualset3
232806	3	428113	15	NULL	NULL	NULL	NULL	18 traumatized patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Free fatty acid ( FFA ) metabolism was studied in 18 traumatized and/or septic patients .
	manualset3
232807	4	428113	15	NULL	NULL	0	NULL	septic patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Free fatty acid ( FFA ) metabolism was studied in 18 traumatized and/or septic patients .
	manualset3
232808	1	428114	15	NULL	NULL	NULL	NULL	mouth	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Restricted mouth opening due to bilateral ankylosis of TMJ and coronoid processes enlargement -- surgical treatment ) .
	manualset3
232809	2	428114	15	NULL	NULL	0	NULL	bilateral ankylosis of TMJ 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Restricted mouth opening due to bilateral ankylosis of TMJ and coronoid processes enlargement -- surgical treatment ) .
	manualset3
232810	3	428114	15	NULL	NULL	0	NULL	coronoid processes enlargement	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Restricted mouth opening due to bilateral ankylosis of TMJ and coronoid processes enlargement -- surgical treatment ) .
	manualset3
232811	4	428114	15	NULL	NULL	0	NULL	surgical treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Restricted mouth opening due to bilateral ankylosis of TMJ and coronoid processes enlargement -- surgical treatment ) .
	manualset3
232818	1	428115	15	NULL	NULL	0	NULL	fractions	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Free fractions of this substance were indistinguishable from unity , indicating little or no protein binding .
	manualset3
232819	2	428115	15	NULL	NULL	0	NULL	substance	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Free fractions of this substance were indistinguishable from unity , indicating little or no protein binding .
	manualset3
232820	3	428115	15	NULL	NULL	0	NULL	unity	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Free fractions of this substance were indistinguishable from unity , indicating little or no protein binding .
	manualset3
232821	4	428115	15	NULL	NULL	NULL	NULL	protein binding	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Free fractions of this substance were indistinguishable from unity , indicating little or no protein binding .
	manualset3
232822	1	428116	15	NULL	NULL	0	NULL	sex steroid binding globulin 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Free sex steroid and sex hormone-binding globulin levels in oligozoospermic men with varicoceles .
	manualset3
232823	2	428116	15	NULL	NULL	0	NULL	sex hormone-binding globulin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Free sex steroid and sex hormone-binding globulin levels in oligozoospermic men with varicoceles .
	manualset3
232824	3	428116	15	NULL	NULL	0	NULL	levels	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Free sex steroid and sex hormone-binding globulin levels in oligozoospermic men with varicoceles .
	manualset3
232825	4	428116	15	NULL	NULL	0	NULL	oligozoospermic men	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Free sex steroid and sex hormone-binding globulin levels in oligozoospermic men with varicoceles .
	manualset3
232826	5	428116	15	NULL	NULL	0	NULL	varicoceles 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Free sex steroid and sex hormone-binding globulin levels in oligozoospermic men with varicoceles .
	manualset3
232827	1	428117	15	NULL	NULL	0	NULL	Frequency	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Frequency dependence of neural response vectors .
	manualset3
232828	2	428117	15	NULL	NULL	0	NULL	dependence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Frequency dependence of neural response vectors .
	manualset3
232829	3	428117	15	NULL	NULL	0	NULL	neural response vectors	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Frequency dependence of neural response vectors .
	manualset3
232830	1	428118	15	NULL	NULL	0	NULL	Frequency	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Frequency of termination of lactations because of mastitis , reproductive problems , or health was similar to frequencies for cattle .
	manualset3
232831	2	428118	15	NULL	NULL	NULL	NULL	termination	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Frequency of termination of lactations because of mastitis , reproductive problems , or health was similar to frequencies for cattle .
	manualset3
232832	4	428118	15	NULL	NULL	NULL	NULL	mastitis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Frequency of termination of lactations because of mastitis , reproductive problems , or health was similar to frequencies for cattle .
	manualset3
232833	5	428118	15	NULL	NULL	NULL	NULL	reproductive problems 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Frequency of termination of lactations because of mastitis , reproductive problems , or health was similar to frequencies for cattle .
	manualset3
232834	6	428118	15	NULL	NULL	NULL	NULL	health	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Frequency of termination of lactations because of mastitis , reproductive problems , or health was similar to frequencies for cattle .
	manualset3
232835	7	428118	15	NULL	NULL	NULL	NULL	similar	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Frequency of termination of lactations because of mastitis , reproductive problems , or health was similar to frequencies for cattle .
	manualset3
232836	8	428118	15	NULL	NULL	NULL	NULL	frequencies	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Frequency of termination of lactations because of mastitis , reproductive problems , or health was similar to frequencies for cattle .
	manualset3
232837	9	428118	15	NULL	NULL	NULL	NULL	cattle	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Frequency of termination of lactations because of mastitis , reproductive problems , or health was similar to frequencies for cattle .
	manualset3
234701	3	428118	15	NULL	NULL	0	NULL	lactations	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Frequency of termination of lactations because of mastitis , reproductive problems , or health was similar to frequencies for cattle .
	manualset3
233063	1	428119	15	NULL	NULL	0	NULL	Frequent calibration checks	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Frequent calibration checks traceable to an independent standard , and adjustment of individual test results , can reduce measurement error .
	manualset3
233064	2	428119	15	NULL	NULL	0	NULL	independent standard	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Frequent calibration checks traceable to an independent standard , and adjustment of individual test results , can reduce measurement error .
	manualset3
233065	3	428119	15	NULL	NULL	0	NULL	adjustment	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Frequent calibration checks traceable to an independent standard , and adjustment of individual test results , can reduce measurement error .
	manualset3
233066	4	428119	15	NULL	NULL	0	NULL	individual test results	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Frequent calibration checks traceable to an independent standard , and adjustment of individual test results , can reduce measurement error .
	manualset3
233067	5	428119	15	NULL	NULL	NULL	NULL	measurement error	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Frequent calibration checks traceable to an independent standard , and adjustment of individual test results , can reduce measurement error .
	manualset3
233068	1	428120	15	NULL	NULL	NULL	NULL	Frequent courses	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Frequent courses of antibiotic therapy are usually required , and some patients may have to receive antibiotics continuously .
	manualset3
233069	2	428120	15	NULL	NULL	0	NULL	antibiotic therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Frequent courses of antibiotic therapy are usually required , and some patients may have to receive antibiotics continuously .
	manualset3
233070	3	428120	15	NULL	NULL	0	NULL	some patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Frequent courses of antibiotic therapy are usually required , and some patients may have to receive antibiotics continuously .
	manualset3
233071	4	428120	15	NULL	NULL	0	NULL	antibiotics	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Frequent courses of antibiotic therapy are usually required , and some patients may have to receive antibiotics continuously .
	manualset3
233074	1	428121	15	NULL	NULL	NULL	NULL	peripheral blood mononuclear cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Freshly isolated and in vitro cytokine-stimulated peripheral blood mononuclear cells from 13 patients with SLE and 10 healthy subjects were analyzed , cytometrically with dual-fluorescence staining , to detect expression of CD80 and CD86 in the CD14 + monocyte population .
	manualset3
233075	2	428121	15	NULL	NULL	NULL	NULL	13 patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Freshly isolated and in vitro cytokine-stimulated peripheral blood mononuclear cells from 13 patients with SLE and 10 healthy subjects were analyzed , cytometrically with dual-fluorescence staining , to detect expression of CD80 and CD86 in the CD14 + monocyte population .
	manualset3
233076	3	428121	15	NULL	NULL	NULL	NULL	SLE	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Freshly isolated and in vitro cytokine-stimulated peripheral blood mononuclear cells from 13 patients with SLE and 10 healthy subjects were analyzed , cytometrically with dual-fluorescence staining , to detect expression of CD80 and CD86 in the CD14 + monocyte population .
	manualset3
233077	4	428121	15	NULL	NULL	NULL	NULL	10 healthy subjects	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Freshly isolated and in vitro cytokine-stimulated peripheral blood mononuclear cells from 13 patients with SLE and 10 healthy subjects were analyzed , cytometrically with dual-fluorescence staining , to detect expression of CD80 and CD86 in the CD14 + monocyte population .
	manualset3
233078	5	428121	15	NULL	NULL	NULL	NULL	dual-fluorescence staining	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Freshly isolated and in vitro cytokine-stimulated peripheral blood mononuclear cells from 13 patients with SLE and 10 healthy subjects were analyzed , cytometrically with dual-fluorescence staining , to detect expression of CD80 and CD86 in the CD14 + monocyte population .
	manualset3
233079	6	428121	15	NULL	NULL	NULL	NULL	expression 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Freshly isolated and in vitro cytokine-stimulated peripheral blood mononuclear cells from 13 patients with SLE and 10 healthy subjects were analyzed , cytometrically with dual-fluorescence staining , to detect expression of CD80 and CD86 in the CD14 + monocyte population .
	manualset3
233080	7	428121	15	NULL	NULL	NULL	NULL	CD80	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Freshly isolated and in vitro cytokine-stimulated peripheral blood mononuclear cells from 13 patients with SLE and 10 healthy subjects were analyzed , cytometrically with dual-fluorescence staining , to detect expression of CD80 and CD86 in the CD14 + monocyte population .
	manualset3
233081	8	428121	15	NULL	NULL	NULL	NULL	CD86	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Freshly isolated and in vitro cytokine-stimulated peripheral blood mononuclear cells from 13 patients with SLE and 10 healthy subjects were analyzed , cytometrically with dual-fluorescence staining , to detect expression of CD80 and CD86 in the CD14 + monocyte population .
	manualset3
233082	9	428121	15	NULL	NULL	NULL	NULL	CD14 + monocyte population	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Freshly isolated and in vitro cytokine-stimulated peripheral blood mononuclear cells from 13 patients with SLE and 10 healthy subjects were analyzed , cytometrically with dual-fluorescence staining , to detect expression of CD80 and CD86 in the CD14 + monocyte population .
	manualset3
233083	1	428122	15	NULL	NULL	0	NULL	chondrocytes	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Freshly isolated chondrocytes , used within 24-48 h of isolation , did not contain actin stress fibers and upregulated SOX9 mRNA in response to hyperosmolarity in the presence and absence of Y27632 .
	manualset3
233084	2	428122	15	NULL	NULL	0	NULL	24-48 h 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Freshly isolated chondrocytes , used within 24-48 h of isolation , did not contain actin stress fibers and upregulated SOX9 mRNA in response to hyperosmolarity in the presence and absence of Y27632 .
	manualset3
233085	3	428122	15	NULL	NULL	0	NULL	 isolation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Freshly isolated chondrocytes , used within 24-48 h of isolation , did not contain actin stress fibers and upregulated SOX9 mRNA in response to hyperosmolarity in the presence and absence of Y27632 .
	manualset3
233086	4	428122	15	NULL	NULL	0	NULL	actin stress fibers	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Freshly isolated chondrocytes , used within 24-48 h of isolation , did not contain actin stress fibers and upregulated SOX9 mRNA in response to hyperosmolarity in the presence and absence of Y27632 .
	manualset3
233087	5	428122	15	NULL	NULL	0	NULL	SOX9 mRNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Freshly isolated chondrocytes , used within 24-48 h of isolation , did not contain actin stress fibers and upregulated SOX9 mRNA in response to hyperosmolarity in the presence and absence of Y27632 .
	manualset3
233088	6	428122	15	NULL	NULL	0	NULL	response	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Freshly isolated chondrocytes , used within 24-48 h of isolation , did not contain actin stress fibers and upregulated SOX9 mRNA in response to hyperosmolarity in the presence and absence of Y27632 .
	manualset3
233089	7	428122	15	NULL	NULL	0	NULL	hyperosmolarity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Freshly isolated chondrocytes , used within 24-48 h of isolation , did not contain actin stress fibers and upregulated SOX9 mRNA in response to hyperosmolarity in the presence and absence of Y27632 .
	manualset3
233090	8	428122	15	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Freshly isolated chondrocytes , used within 24-48 h of isolation , did not contain actin stress fibers and upregulated SOX9 mRNA in response to hyperosmolarity in the presence and absence of Y27632 .
	manualset3
233091	9	428122	15	NULL	NULL	0	NULL	absence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Freshly isolated chondrocytes , used within 24-48 h of isolation , did not contain actin stress fibers and upregulated SOX9 mRNA in response to hyperosmolarity in the presence and absence of Y27632 .
	manualset3
233092	10	428122	15	NULL	NULL	NULL	NULL	Y27632	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Freshly isolated chondrocytes , used within 24-48 h of isolation , did not contain actin stress fibers and upregulated SOX9 mRNA in response to hyperosmolarity in the presence and absence of Y27632 .
	manualset3
233093	1	428123	15	NULL	NULL	0	NULL	Friedreich ataxia ( FA )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Friedreich ataxia ( FA ) is caused by decreased frataxin expression that results in mitochondrial iron ( Fe ) overload .
	manualset3
233094	2	428123	15	NULL	NULL	0	NULL	frataxin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Friedreich ataxia ( FA ) is caused by decreased frataxin expression that results in mitochondrial iron ( Fe ) overload .
	manualset3
233095	3	428123	15	NULL	NULL	0	NULL	expression 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Friedreich ataxia ( FA ) is caused by decreased frataxin expression that results in mitochondrial iron ( Fe ) overload .
	manualset3
233096	4	428123	15	NULL	NULL	0	NULL	mitochondrial iron ( Fe )	Atom												NULL		0	NULL	NULL	NULL	NULL	NULL	Friedreich ataxia ( FA ) is caused by decreased frataxin expression that results in mitochondrial iron ( Fe ) overload .
	manualset3
233097	1	428124	15	NULL	NULL	0	NULL	( 15 ) N relaxation experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	From ( 15 ) N relaxation experiments , an increase in the overall correlation time of cytochrome b ( 5 ) in the presence of myoglobin is observed , confirming that complex formation is occurring .
	manualset3
233098	2	428124	15	NULL	NULL	0	NULL	increase	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	From ( 15 ) N relaxation experiments , an increase in the overall correlation time of cytochrome b ( 5 ) in the presence of myoglobin is observed , confirming that complex formation is occurring .
	manualset3
233099	3	428124	15	NULL	NULL	NULL	NULL	correlation time	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From ( 15 ) N relaxation experiments , an increase in the overall correlation time of cytochrome b ( 5 ) in the presence of myoglobin is observed , confirming that complex formation is occurring .
	manualset3
233100	4	428124	15	NULL	NULL	0	NULL	cytochrome b ( 5 ) 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	From ( 15 ) N relaxation experiments , an increase in the overall correlation time of cytochrome b ( 5 ) in the presence of myoglobin is observed , confirming that complex formation is occurring .
	manualset3
233101	5	428124	15	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	From ( 15 ) N relaxation experiments , an increase in the overall correlation time of cytochrome b ( 5 ) in the presence of myoglobin is observed , confirming that complex formation is occurring .
	manualset3
233102	6	428124	15	NULL	NULL	0	NULL	myoglobin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	From ( 15 ) N relaxation experiments , an increase in the overall correlation time of cytochrome b ( 5 ) in the presence of myoglobin is observed , confirming that complex formation is occurring .
	manualset3
233103	7	428124	15	NULL	NULL	NULL	NULL	complex formation	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From ( 15 ) N relaxation experiments , an increase in the overall correlation time of cytochrome b ( 5 ) in the presence of myoglobin is observed , confirming that complex formation is occurring .
	manualset3
233104	1	428125	15	NULL	NULL	0	NULL	1939 onwards	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	From 1939 onwards , the young chest surgeons were confronted with war wounds of the heart and great vessels .
	manualset3
233105	2	428125	15	NULL	NULL	0	NULL	young chest surgeons	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	From 1939 onwards , the young chest surgeons were confronted with war wounds of the heart and great vessels .
	manualset3
233106	3	428125	15	NULL	NULL	0	NULL	war wounds	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	From 1939 onwards , the young chest surgeons were confronted with war wounds of the heart and great vessels .
	manualset3
233107	4	428125	15	NULL	NULL	0	NULL	heart	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	From 1939 onwards , the young chest surgeons were confronted with war wounds of the heart and great vessels .
	manualset3
233108	5	428125	15	NULL	NULL	0	NULL	vessels 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	From 1939 onwards , the young chest surgeons were confronted with war wounds of the heart and great vessels .
	manualset3
233109	1	428126	15	NULL	NULL	0	NULL	1961 to 1989	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	From 1961 to 1989 , 67 patients underwent various surgical procedures for psoas abscess .
	manualset3
233110	2	428126	15	NULL	NULL	0	NULL	67 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	From 1961 to 1989 , 67 patients underwent various surgical procedures for psoas abscess .
	manualset3
233111	3	428126	15	NULL	NULL	0	NULL	surgical procedures 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	From 1961 to 1989 , 67 patients underwent various surgical procedures for psoas abscess .
	manualset3
233112	4	428126	15	NULL	NULL	0	NULL	psoas abscess	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	From 1961 to 1989 , 67 patients underwent various surgical procedures for psoas abscess .
	manualset3
233113	1	428127	15	NULL	NULL	0	NULL	From 1969 through 1972	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	From 1969 through 1972 , a nationwide search for cases of Guillain-Barr syndrome ( GBS ) is Israel revealed 89 patients .
	manualset3
233114	2	428127	15	NULL	NULL	0	NULL	search	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	From 1969 through 1972 , a nationwide search for cases of Guillain-Barr syndrome ( GBS ) is Israel revealed 89 patients .
	manualset3
233115	3	428127	15	NULL	NULL	0	NULL	cases 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	From 1969 through 1972 , a nationwide search for cases of Guillain-Barr syndrome ( GBS ) is Israel revealed 89 patients .
	manualset3
233116	4	428127	15	NULL	NULL	NULL	NULL	Guillain-Barr syndrome ( GBS ) 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From 1969 through 1972 , a nationwide search for cases of Guillain-Barr syndrome ( GBS ) is Israel revealed 89 patients .
	manualset3
233117	5	428127	15	NULL	NULL	0	NULL	Israel	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	From 1969 through 1972 , a nationwide search for cases of Guillain-Barr syndrome ( GBS ) is Israel revealed 89 patients .
	manualset3
233118	6	428127	15	NULL	NULL	0	NULL	89 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	From 1969 through 1972 , a nationwide search for cases of Guillain-Barr syndrome ( GBS ) is Israel revealed 89 patients .
	manualset3
233119	1	428128	15	NULL	NULL	0	NULL	From 2003-2004 to 2005-2006 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	From 2003-2004 to 2005-2006 , total and targeted antibiotic consumption , respectively , decreased by 23 % and 54 % , and the incidence of n-CDAD decreased by 60 % .
	manualset3
233120	2	428128	15	NULL	NULL	NULL	NULL	antibiotic consumption	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From 2003-2004 to 2005-2006 , total and targeted antibiotic consumption , respectively , decreased by 23 % and 54 % , and the incidence of n-CDAD decreased by 60 % .
	manualset3
233121	3	428128	15	NULL	NULL	0	NULL	23 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	From 2003-2004 to 2005-2006 , total and targeted antibiotic consumption , respectively , decreased by 23 % and 54 % , and the incidence of n-CDAD decreased by 60 % .
	manualset3
233122	4	428128	15	NULL	NULL	0	NULL	54 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	From 2003-2004 to 2005-2006 , total and targeted antibiotic consumption , respectively , decreased by 23 % and 54 % , and the incidence of n-CDAD decreased by 60 % .
	manualset3
233123	5	428128	15	NULL	NULL	0	NULL	incidence	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	From 2003-2004 to 2005-2006 , total and targeted antibiotic consumption , respectively , decreased by 23 % and 54 % , and the incidence of n-CDAD decreased by 60 % .
	manualset3
233124	6	428128	15	NULL	NULL	0	NULL	n-CDAD	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	From 2003-2004 to 2005-2006 , total and targeted antibiotic consumption , respectively , decreased by 23 % and 54 % , and the incidence of n-CDAD decreased by 60 % .
	manualset3
233125	7	428128	15	NULL	NULL	0	NULL	60 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	From 2003-2004 to 2005-2006 , total and targeted antibiotic consumption , respectively , decreased by 23 % and 54 % , and the incidence of n-CDAD decreased by 60 % .
	manualset3
233126	1	428129	15	NULL	NULL	0	NULL	6-12 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	From 6-12 h after exposure , there was a substantial increase in the percentage of cells undergoing S phase arrest and apoptosis .
	manualset3
233127	2	428129	15	NULL	NULL	0	NULL	exposure	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	From 6-12 h after exposure , there was a substantial increase in the percentage of cells undergoing S phase arrest and apoptosis .
	manualset3
233128	3	428129	15	NULL	NULL	NULL	NULL	increase	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From 6-12 h after exposure , there was a substantial increase in the percentage of cells undergoing S phase arrest and apoptosis .
	manualset3
233129	5	428129	15	NULL	NULL	NULL	NULL	cells	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From 6-12 h after exposure , there was a substantial increase in the percentage of cells undergoing S phase arrest and apoptosis .
	manualset3
233130	6	428129	15	NULL	NULL	NULL	NULL	S phase arrest	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From 6-12 h after exposure , there was a substantial increase in the percentage of cells undergoing S phase arrest and apoptosis .
	manualset3
233131	7	428129	15	NULL	NULL	NULL	NULL	apoptosis	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From 6-12 h after exposure , there was a substantial increase in the percentage of cells undergoing S phase arrest and apoptosis .
	manualset3
234713	4	428129	15	NULL	NULL	0	NULL	percentage	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	From 6-12 h after exposure , there was a substantial increase in the percentage of cells undergoing S phase arrest and apoptosis .
	manualset3
233132	1	428130	15	NULL	NULL	0	NULL	From April 2003 through June 2004	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	From April 2003 through June 2004 , 53 hospitals reported 290 cases of A. baumannii infection or colonization ; 275 isolates were bla ( VEB-1 ) - positive and clonally related .
	manualset3
233133	2	428130	15	NULL	NULL	0	NULL	53 hospitals	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	From April 2003 through June 2004 , 53 hospitals reported 290 cases of A. baumannii infection or colonization ; 275 isolates were bla ( VEB-1 ) - positive and clonally related .
	manualset3
233134	3	428130	15	NULL	NULL	0	NULL	290 cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	From April 2003 through June 2004 , 53 hospitals reported 290 cases of A. baumannii infection or colonization ; 275 isolates were bla ( VEB-1 ) - positive and clonally related .
	manualset3
233135	4	428130	15	NULL	NULL	0	NULL	A. baumannii infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	From April 2003 through June 2004 , 53 hospitals reported 290 cases of A. baumannii infection or colonization ; 275 isolates were bla ( VEB-1 ) - positive and clonally related .
	manualset3
233136	5	428130	15	NULL	NULL	0	NULL	A. baumannii colonization	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	From April 2003 through June 2004 , 53 hospitals reported 290 cases of A. baumannii infection or colonization ; 275 isolates were bla ( VEB-1 ) - positive and clonally related .
	manualset3
233137	6	428130	15	NULL	NULL	NULL	NULL	275 isolates	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From April 2003 through June 2004 , 53 hospitals reported 290 cases of A. baumannii infection or colonization ; 275 isolates were bla ( VEB-1 ) - positive and clonally related .
	manualset3
233138	7	428130	15	NULL	NULL	0	NULL	bla ( VEB-1 )	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	From April 2003 through June 2004 , 53 hospitals reported 290 cases of A. baumannii infection or colonization ; 275 isolates were bla ( VEB-1 ) - positive and clonally related .
	manualset3
233140	1	428131	15	NULL	NULL	NULL	NULL	January 1984 through November 1985	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From January 1984 through November 1985 , 31 clinical cases of hepatitis B occurred among attendees of a weight reduction clinic ( clinic 1 ) .
	manualset3
233141	2	428131	15	NULL	NULL	0	NULL	31 clinical cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	From January 1984 through November 1985 , 31 clinical cases of hepatitis B occurred among attendees of a weight reduction clinic ( clinic 1 ) .
	manualset3
233142	3	428131	15	NULL	NULL	0	NULL	hepatitis B	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	From January 1984 through November 1985 , 31 clinical cases of hepatitis B occurred among attendees of a weight reduction clinic ( clinic 1 ) .
	manualset3
233143	4	428131	15	NULL	NULL	0	NULL	attendees 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	From January 1984 through November 1985 , 31 clinical cases of hepatitis B occurred among attendees of a weight reduction clinic ( clinic 1 ) .
	manualset3
233144	5	428131	15	NULL	NULL	NULL	NULL	weight reduction clinic 	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From January 1984 through November 1985 , 31 clinical cases of hepatitis B occurred among attendees of a weight reduction clinic ( clinic 1 ) .
	manualset3
233145	6	428131	15	NULL	NULL	0	NULL	( clinic 1 )	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	From January 1984 through November 1985 , 31 clinical cases of hepatitis B occurred among attendees of a weight reduction clinic ( clinic 1 ) .
	manualset3
233146	1	428132	15	NULL	NULL	NULL	NULL	May to August	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From May to August , the plants in treatment cutting had more leaves and tender stems but less old stems , and in September , their inedible part for livestock was 69.26 % of the total biomass while that in treatment un-cutting was 77.79 % .
	manualset3
233147	2	428132	15	NULL	NULL	0	NULL	 plants	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	From May to August , the plants in treatment cutting had more leaves and tender stems but less old stems , and in September , their inedible part for livestock was 69.26 % of the total biomass while that in treatment un-cutting was 77.79 % .
	manualset3
233148	3	428132	15	NULL	NULL	NULL	NULL	treatment 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From May to August , the plants in treatment cutting had more leaves and tender stems but less old stems , and in September , their inedible part for livestock was 69.26 % of the total biomass while that in treatment un-cutting was 77.79 % .
	manualset3
233149	4	428132	15	NULL	NULL	0	NULL	leaves	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	From May to August , the plants in treatment cutting had more leaves and tender stems but less old stems , and in September , their inedible part for livestock was 69.26 % of the total biomass while that in treatment un-cutting was 77.79 % .
	manualset3
233150	5	428132	15	NULL	NULL	0	NULL	stems	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	From May to August , the plants in treatment cutting had more leaves and tender stems but less old stems , and in September , their inedible part for livestock was 69.26 % of the total biomass while that in treatment un-cutting was 77.79 % .
	manualset3
233151	6	428132	15	NULL	NULL	0	NULL	stems	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	From May to August , the plants in treatment cutting had more leaves and tender stems but less old stems , and in September , their inedible part for livestock was 69.26 % of the total biomass while that in treatment un-cutting was 77.79 % .
	manualset3
233152	7	428132	15	NULL	NULL	0	NULL	September	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	From May to August , the plants in treatment cutting had more leaves and tender stems but less old stems , and in September , their inedible part for livestock was 69.26 % of the total biomass while that in treatment un-cutting was 77.79 % .
	manualset3
233153	8	428132	15	NULL	NULL	0	NULL	inedible part	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	From May to August , the plants in treatment cutting had more leaves and tender stems but less old stems , and in September , their inedible part for livestock was 69.26 % of the total biomass while that in treatment un-cutting was 77.79 % .
	manualset3
233154	9	428132	15	NULL	NULL	NULL	NULL	livestock	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From May to August , the plants in treatment cutting had more leaves and tender stems but less old stems , and in September , their inedible part for livestock was 69.26 % of the total biomass while that in treatment un-cutting was 77.79 % .
	manualset3
233155	10	428132	15	NULL	NULL	0	NULL	 69.26 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	From May to August , the plants in treatment cutting had more leaves and tender stems but less old stems , and in September , their inedible part for livestock was 69.26 % of the total biomass while that in treatment un-cutting was 77.79 % .
	manualset3
233156	11	428132	15	NULL	NULL	0	NULL	biomass 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	From May to August , the plants in treatment cutting had more leaves and tender stems but less old stems , and in September , their inedible part for livestock was 69.26 % of the total biomass while that in treatment un-cutting was 77.79 % .
	manualset3
233157	12	428132	15	NULL	NULL	0	NULL	treatment un-cutting	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	From May to August , the plants in treatment cutting had more leaves and tender stems but less old stems , and in September , their inedible part for livestock was 69.26 % of the total biomass while that in treatment un-cutting was 77.79 % .
	manualset3
233158	13	428132	15	NULL	NULL	0	NULL	77.79 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	From May to August , the plants in treatment cutting had more leaves and tender stems but less old stems , and in September , their inedible part for livestock was 69.26 % of the total biomass while that in treatment un-cutting was 77.79 % .
	manualset3
233229	1	428133	15	NULL	NULL	NULL	NULL	October 2006 to October 2007	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From October 2006 to October 2007 , a total of 34 patients ( age range , 22 to 42 years ) with kyphosis and a thoracic curvature between 45 and 88 were examined prospectively at a sports medicine clinic belonging to National Iranian Oil Company ( N.I.O.C. ) .
	manualset3
233230	2	428133	15	NULL	NULL	0	NULL	34 patients 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	From October 2006 to October 2007 , a total of 34 patients ( age range , 22 to 42 years ) with kyphosis and a thoracic curvature between 45 and 88 were examined prospectively at a sports medicine clinic belonging to National Iranian Oil Company ( N.I.O.C. ) .
	manualset3
233231	3	428133	15	NULL	NULL	NULL	NULL	age range	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From October 2006 to October 2007 , a total of 34 patients ( age range , 22 to 42 years ) with kyphosis and a thoracic curvature between 45 and 88 were examined prospectively at a sports medicine clinic belonging to National Iranian Oil Company ( N.I.O.C. ) .
	manualset3
233232	5	428133	15	NULL	NULL	NULL	NULL	kyphosis	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From October 2006 to October 2007 , a total of 34 patients ( age range , 22 to 42 years ) with kyphosis and a thoracic curvature between 45 and 88 were examined prospectively at a sports medicine clinic belonging to National Iranian Oil Company ( N.I.O.C. ) .
	manualset3
233233	6	428133	15	NULL	NULL	NULL	NULL	thoracic curvature	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From October 2006 to October 2007 , a total of 34 patients ( age range , 22 to 42 years ) with kyphosis and a thoracic curvature between 45 and 88 were examined prospectively at a sports medicine clinic belonging to National Iranian Oil Company ( N.I.O.C. ) .
	manualset3
233234	7	428133	15	NULL	NULL	NULL	NULL	45 and 88	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From October 2006 to October 2007 , a total of 34 patients ( age range , 22 to 42 years ) with kyphosis and a thoracic curvature between 45 and 88 were examined prospectively at a sports medicine clinic belonging to National Iranian Oil Company ( N.I.O.C. ) .
	manualset3
233235	8	428133	15	NULL	NULL	NULL	NULL	sports medicine clinic	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From October 2006 to October 2007 , a total of 34 patients ( age range , 22 to 42 years ) with kyphosis and a thoracic curvature between 45 and 88 were examined prospectively at a sports medicine clinic belonging to National Iranian Oil Company ( N.I.O.C. ) .
	manualset3
233236	9	428133	15	NULL	NULL	NULL	NULL	National Iranian Oil Company ( N.I.O.C. )	Facility												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From October 2006 to October 2007 , a total of 34 patients ( age range , 22 to 42 years ) with kyphosis and a thoracic curvature between 45 and 88 were examined prospectively at a sports medicine clinic belonging to National Iranian Oil Company ( N.I.O.C. ) .
	manualset3
234738	4	428133	15	NULL	NULL	0	NULL	22 to 42 years	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	From October 2006 to October 2007 , a total of 34 patients ( age range , 22 to 42 years ) with kyphosis and a thoracic curvature between 45 and 88 were examined prospectively at a sports medicine clinic belonging to National Iranian Oil Company ( N.I.O.C. ) .
	manualset3
233237	1	428134	15	NULL	NULL	0	NULL	Results 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Results of the first three years of operation of the emergency medical assistance service ( SAMU ) in Yaounde , Cameroon ) .
	manualset3
233238	2	428134	15	NULL	NULL	0	NULL	first three years	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	( Results of the first three years of operation of the emergency medical assistance service ( SAMU ) in Yaounde , Cameroon ) .
	manualset3
233239	3	428134	15	NULL	NULL	0	NULL	operation 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Results of the first three years of operation of the emergency medical assistance service ( SAMU ) in Yaounde , Cameroon ) .
	manualset3
233240	4	428134	15	NULL	NULL	NULL	NULL	emergency medical assistance service ( SAMU )	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Results of the first three years of operation of the emergency medical assistance service ( SAMU ) in Yaounde , Cameroon ) .
	manualset3
233241	5	428134	15	NULL	NULL	0	NULL	Yaounde , Cameroon	ProperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	( Results of the first three years of operation of the emergency medical assistance service ( SAMU ) in Yaounde , Cameroon ) .
	manualset3
233242	1	428135	15	NULL	NULL	0	NULL	cultural  perspective	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	From a cultural and social perspective , Latinos represent a wide variety of national origins and ethnic and cultural groups , with a full spectrum of social class .
	manualset3
233243	2	428135	15	NULL	NULL	0	NULL	social perspective	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	From a cultural and social perspective , Latinos represent a wide variety of national origins and ethnic and cultural groups , with a full spectrum of social class .
	manualset3
233244	3	428135	15	NULL	NULL	0	NULL	Latinos	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	From a cultural and social perspective , Latinos represent a wide variety of national origins and ethnic and cultural groups , with a full spectrum of social class .
	manualset3
233245	4	428135	15	NULL	NULL	0	NULL	variety	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	From a cultural and social perspective , Latinos represent a wide variety of national origins and ethnic and cultural groups , with a full spectrum of social class .
	manualset3
233246	5	428135	15	NULL	NULL	0	NULL	national origins	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	From a cultural and social perspective , Latinos represent a wide variety of national origins and ethnic and cultural groups , with a full spectrum of social class .
	manualset3
233247	6	428135	15	NULL	NULL	0	NULL	ethnic groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	From a cultural and social perspective , Latinos represent a wide variety of national origins and ethnic and cultural groups , with a full spectrum of social class .
	manualset3
233248	7	428135	15	NULL	NULL	0	NULL	cultural groups	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	From a cultural and social perspective , Latinos represent a wide variety of national origins and ethnic and cultural groups , with a full spectrum of social class .
	manualset3
233249	8	428135	15	NULL	NULL	0	NULL	spectrum	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	From a cultural and social perspective , Latinos represent a wide variety of national origins and ethnic and cultural groups , with a full spectrum of social class .
	manualset3
233250	9	428135	15	NULL	NULL	0	NULL	social class	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	From a cultural and social perspective , Latinos represent a wide variety of national origins and ethnic and cultural groups , with a full spectrum of social class .
	manualset3
233251	1	428136	15	NULL	NULL	0	NULL	angular dependent study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	From a detailed angular and temperature dependent study of the de Haas-van Alphen effect we determine the electronic structure and demonstrate that the electron masses are very light , m * approximately 1.2 me .
	manualset3
233252	2	428136	15	NULL	NULL	0	NULL	temperature dependent study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	From a detailed angular and temperature dependent study of the de Haas-van Alphen effect we determine the electronic structure and demonstrate that the electron masses are very light , m * approximately 1.2 me .
	manualset3
233253	3	428136	15	NULL	NULL	NULL	NULL	de Haas-van Alphen effect	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From a detailed angular and temperature dependent study of the de Haas-van Alphen effect we determine the electronic structure and demonstrate that the electron masses are very light , m * approximately 1.2 me .
	manualset3
233254	4	428136	15	NULL	NULL	NULL	NULL	electronic structure	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From a detailed angular and temperature dependent study of the de Haas-van Alphen effect we determine the electronic structure and demonstrate that the electron masses are very light , m * approximately 1.2 me .
	manualset3
233255	5	428136	15	NULL	NULL	0	NULL	electron masses	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	From a detailed angular and temperature dependent study of the de Haas-van Alphen effect we determine the electronic structure and demonstrate that the electron masses are very light , m * approximately 1.2 me .
	manualset3
233256	6	428136	15	NULL	NULL	0	NULL	m * approximately 1.2 me	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	From a detailed angular and temperature dependent study of the de Haas-van Alphen effect we determine the electronic structure and demonstrate that the electron masses are very light , m * approximately 1.2 me .
	manualset3
233257	1	428137	15	NULL	NULL	0	NULL	retrospective study 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	From a retrospective study of 132 patients it appears that the incidence of this troublesome complication can be reduced after osteotomy with external fixation by using a technique of making consecutive drill holes of increasing diameter followed by osteoclasis .
	manualset3
233258	2	428137	15	NULL	NULL	0	NULL	132 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	From a retrospective study of 132 patients it appears that the incidence of this troublesome complication can be reduced after osteotomy with external fixation by using a technique of making consecutive drill holes of increasing diameter followed by osteoclasis .
	manualset3
233259	3	428137	15	NULL	NULL	0	NULL	incidence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	From a retrospective study of 132 patients it appears that the incidence of this troublesome complication can be reduced after osteotomy with external fixation by using a technique of making consecutive drill holes of increasing diameter followed by osteoclasis .
	manualset3
233260	4	428137	15	NULL	NULL	0	NULL	troublesome complication	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	From a retrospective study of 132 patients it appears that the incidence of this troublesome complication can be reduced after osteotomy with external fixation by using a technique of making consecutive drill holes of increasing diameter followed by osteoclasis .
	manualset3
233261	5	428137	15	NULL	NULL	0	NULL	osteotomy 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	From a retrospective study of 132 patients it appears that the incidence of this troublesome complication can be reduced after osteotomy with external fixation by using a technique of making consecutive drill holes of increasing diameter followed by osteoclasis .
	manualset3
233262	6	428137	15	NULL	NULL	0	NULL	external fixation	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	From a retrospective study of 132 patients it appears that the incidence of this troublesome complication can be reduced after osteotomy with external fixation by using a technique of making consecutive drill holes of increasing diameter followed by osteoclasis .
	manualset3
233263	7	428137	15	NULL	NULL	NULL	NULL	technique	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From a retrospective study of 132 patients it appears that the incidence of this troublesome complication can be reduced after osteotomy with external fixation by using a technique of making consecutive drill holes of increasing diameter followed by osteoclasis .
	manualset3
233264	8	428137	15	NULL	NULL	NULL	NULL	making consecutive drill holes 	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From a retrospective study of 132 patients it appears that the incidence of this troublesome complication can be reduced after osteotomy with external fixation by using a technique of making consecutive drill holes of increasing diameter followed by osteoclasis .
	manualset3
233265	9	428137	15	NULL	NULL	0	NULL	diameter 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	From a retrospective study of 132 patients it appears that the incidence of this troublesome complication can be reduced after osteotomy with external fixation by using a technique of making consecutive drill holes of increasing diameter followed by osteoclasis .
	manualset3
233266	10	428137	15	NULL	NULL	0	NULL	osteoclasis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	From a retrospective study of 132 patients it appears that the incidence of this troublesome complication can be reduced after osteotomy with external fixation by using a technique of making consecutive drill holes of increasing diameter followed by osteoclasis .
	manualset3
233311	1	428138	15	NULL	NULL	0	NULL	structured history	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	From a structured history of 32 current smokers seen in the pulmonary function laboratory of a community hospital , we determined the number of cigarettes they smoked in 24 h. We also asked them to estimate their cigarette butt lengths from a visual model and to collect all cigarette butts over the next 24 h and mail them to us .
	manualset3
233312	2	428138	15	NULL	NULL	0	NULL	32 current smokers 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	From a structured history of 32 current smokers seen in the pulmonary function laboratory of a community hospital , we determined the number of cigarettes they smoked in 24 h. We also asked them to estimate their cigarette butt lengths from a visual model and to collect all cigarette butts over the next 24 h and mail them to us .
	manualset3
233313	3	428138	15	NULL	NULL	0	NULL	pulmonary function laboratory 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	From a structured history of 32 current smokers seen in the pulmonary function laboratory of a community hospital , we determined the number of cigarettes they smoked in 24 h. We also asked them to estimate their cigarette butt lengths from a visual model and to collect all cigarette butts over the next 24 h and mail them to us .
	manualset3
233314	4	428138	15	NULL	NULL	0	NULL	community hospital	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	From a structured history of 32 current smokers seen in the pulmonary function laboratory of a community hospital , we determined the number of cigarettes they smoked in 24 h. We also asked them to estimate their cigarette butt lengths from a visual model and to collect all cigarette butts over the next 24 h and mail them to us .
	manualset3
233315	5	428138	15	NULL	NULL	0	NULL	number 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	From a structured history of 32 current smokers seen in the pulmonary function laboratory of a community hospital , we determined the number of cigarettes they smoked in 24 h. We also asked them to estimate their cigarette butt lengths from a visual model and to collect all cigarette butts over the next 24 h and mail them to us .
	manualset3
233316	6	428138	15	NULL	NULL	0	NULL	cigarettes	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	From a structured history of 32 current smokers seen in the pulmonary function laboratory of a community hospital , we determined the number of cigarettes they smoked in 24 h. We also asked them to estimate their cigarette butt lengths from a visual model and to collect all cigarette butts over the next 24 h and mail them to us .
	manualset3
233317	7	428138	15	NULL	NULL	0	NULL	24 h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	From a structured history of 32 current smokers seen in the pulmonary function laboratory of a community hospital , we determined the number of cigarettes they smoked in 24 h. We also asked them to estimate their cigarette butt lengths from a visual model and to collect all cigarette butts over the next 24 h and mail them to us .
	manualset3
233318	8	428138	15	NULL	NULL	0	NULL	cigarette butt lengths	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	From a structured history of 32 current smokers seen in the pulmonary function laboratory of a community hospital , we determined the number of cigarettes they smoked in 24 h. We also asked them to estimate their cigarette butt lengths from a visual model and to collect all cigarette butts over the next 24 h and mail them to us .
	manualset3
233319	9	428138	15	NULL	NULL	0	NULL	visual model	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	From a structured history of 32 current smokers seen in the pulmonary function laboratory of a community hospital , we determined the number of cigarettes they smoked in 24 h. We also asked them to estimate their cigarette butt lengths from a visual model and to collect all cigarette butts over the next 24 h and mail them to us .
	manualset3
233320	10	428138	15	NULL	NULL	0	NULL	cigarette butts	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	From a structured history of 32 current smokers seen in the pulmonary function laboratory of a community hospital , we determined the number of cigarettes they smoked in 24 h. We also asked them to estimate their cigarette butt lengths from a visual model and to collect all cigarette butts over the next 24 h and mail them to us .
	manualset3
233321	11	428138	15	NULL	NULL	0	NULL	24 h 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	From a structured history of 32 current smokers seen in the pulmonary function laboratory of a community hospital , we determined the number of cigarettes they smoked in 24 h. We also asked them to estimate their cigarette butt lengths from a visual model and to collect all cigarette butts over the next 24 h and mail them to us .
	manualset3
233322	1	428139	15	NULL	NULL	0	NULL	antiretroviral drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	From antiretroviral drugs to antifungal , antibacterial and antitumor agents based on aspartic protease inhibitors .
	manualset3
233323	2	428139	15	NULL	NULL	0	NULL	antifungal agents	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	From antiretroviral drugs to antifungal , antibacterial and antitumor agents based on aspartic protease inhibitors .
	manualset3
233324	3	428139	15	NULL	NULL	0	NULL	antibacterial agents	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	From antiretroviral drugs to antifungal , antibacterial and antitumor agents based on aspartic protease inhibitors .
	manualset3
233325	4	428139	15	NULL	NULL	0	NULL	antitumor agents	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	From antiretroviral drugs to antifungal , antibacterial and antitumor agents based on aspartic protease inhibitors .
	manualset3
233326	5	428139	15	NULL	NULL	NULL	NULL	aspartic protease inhibitors	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From antiretroviral drugs to antifungal , antibacterial and antitumor agents based on aspartic protease inhibitors .
	manualset3
233327	1	428140	15	NULL	NULL	0	NULL	cell death	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	From cell death to neuronal regeneration : building a new brain after traumatic brain injury .
	manualset3
233328	2	428140	15	NULL	NULL	0	NULL	neuronal regeneration	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	From cell death to neuronal regeneration : building a new brain after traumatic brain injury .
	manualset3
233329	3	428140	15	NULL	NULL	0	NULL	brain 	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	From cell death to neuronal regeneration : building a new brain after traumatic brain injury .
	manualset3
233330	4	428140	15	NULL	NULL	0	NULL	traumatic brain injury	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	From cell death to neuronal regeneration : building a new brain after traumatic brain injury .
	manualset3
233331	1	428141	15	NULL	NULL	0	NULL	comparisons	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	From comparisons between results obtained with various genera of lagomorphs , and hypothetical scheme is proposed for the evolution of the Cgamma gene on the basis of the series allotypes .
	manualset3
233332	2	428141	15	NULL	NULL	NULL	NULL	 results	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From comparisons between results obtained with various genera of lagomorphs , and hypothetical scheme is proposed for the evolution of the Cgamma gene on the basis of the series allotypes .
	manualset3
233333	3	428141	15	NULL	NULL	0	NULL	genera of lagomorphs 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	From comparisons between results obtained with various genera of lagomorphs , and hypothetical scheme is proposed for the evolution of the Cgamma gene on the basis of the series allotypes .
	manualset3
233334	4	428141	15	NULL	NULL	0	NULL	hypothetical scheme	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	From comparisons between results obtained with various genera of lagomorphs , and hypothetical scheme is proposed for the evolution of the Cgamma gene on the basis of the series allotypes .
	manualset3
233335	5	428141	15	NULL	NULL	0	NULL	evolution 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	From comparisons between results obtained with various genera of lagomorphs , and hypothetical scheme is proposed for the evolution of the Cgamma gene on the basis of the series allotypes .
	manualset3
233336	6	428141	15	NULL	NULL	0	NULL	Cgamma gene	Gene												NULL		0	NULL	NULL	NULL	NULL	NULL	From comparisons between results obtained with various genera of lagomorphs , and hypothetical scheme is proposed for the evolution of the Cgamma gene on the basis of the series allotypes .
	manualset3
233337	7	428141	15	NULL	NULL	0	NULL	basis 	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	From comparisons between results obtained with various genera of lagomorphs , and hypothetical scheme is proposed for the evolution of the Cgamma gene on the basis of the series allotypes .
	manualset3
233338	8	428141	15	NULL	NULL	0	NULL	series allotypes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	From comparisons between results obtained with various genera of lagomorphs , and hypothetical scheme is proposed for the evolution of the Cgamma gene on the basis of the series allotypes .
	manualset3
233339	1	428142	15	NULL	NULL	NULL	NULL	computational evolutionary structure searches	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From computational evolutionary structure searches , we find a sequence of new stable and meta-stable structures for the ground state of ice in the 1-5 TPa ( 10 to 50 Mbar ) regime , in the static approximation .
	manualset3
233341	2	428142	15	NULL	NULL	NULL	NULL	sequence	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From computational evolutionary structure searches , we find a sequence of new stable and meta-stable structures for the ground state of ice in the 1-5 TPa ( 10 to 50 Mbar ) regime , in the static approximation .
	manualset3
233342	3	428142	15	NULL	NULL	NULL	NULL	new stable structures	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From computational evolutionary structure searches , we find a sequence of new stable and meta-stable structures for the ground state of ice in the 1-5 TPa ( 10 to 50 Mbar ) regime , in the static approximation .
	manualset3
233343	4	428142	15	NULL	NULL	NULL	NULL	meta-stable structures	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From computational evolutionary structure searches , we find a sequence of new stable and meta-stable structures for the ground state of ice in the 1-5 TPa ( 10 to 50 Mbar ) regime , in the static approximation .
	manualset3
233344	5	428142	15	NULL	NULL	NULL	NULL	ground state	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From computational evolutionary structure searches , we find a sequence of new stable and meta-stable structures for the ground state of ice in the 1-5 TPa ( 10 to 50 Mbar ) regime , in the static approximation .
	manualset3
233345	6	428142	15	NULL	NULL	NULL	NULL	ice	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From computational evolutionary structure searches , we find a sequence of new stable and meta-stable structures for the ground state of ice in the 1-5 TPa ( 10 to 50 Mbar ) regime , in the static approximation .
	manualset3
233346	7	428142	15	NULL	NULL	NULL	NULL	1-5 TPa ( 10 to 50 Mbar ) regime	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From computational evolutionary structure searches , we find a sequence of new stable and meta-stable structures for the ground state of ice in the 1-5 TPa ( 10 to 50 Mbar ) regime , in the static approximation .
	manualset3
233348	8	428142	15	NULL	NULL	NULL	NULL	static approximation	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From computational evolutionary structure searches , we find a sequence of new stable and meta-stable structures for the ground state of ice in the 1-5 TPa ( 10 to 50 Mbar ) regime , in the static approximation .
	manualset3
233349	1	428143	15	NULL	NULL	NULL	NULL	Results	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Results of treatment of leg paraspasm cases following longitudinal frontal myelotomy ) .
	manualset3
233350	2	428143	15	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Results of treatment of leg paraspasm cases following longitudinal frontal myelotomy ) .
	manualset3
233351	3	428143	15	NULL	NULL	0	NULL	 leg paraspasm	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Results of treatment of leg paraspasm cases following longitudinal frontal myelotomy ) .
	manualset3
233352	4	428143	15	NULL	NULL	0	NULL	cases	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Results of treatment of leg paraspasm cases following longitudinal frontal myelotomy ) .
	manualset3
233353	5	428143	15	NULL	NULL	0	NULL	longitudinal frontal myelotomy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Results of treatment of leg paraspasm cases following longitudinal frontal myelotomy ) .
	manualset3
233354	1	428144	15	NULL	NULL	0	NULL	day 50 to 132	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	From day 50 to 132 of pregnancy ( tissue collection day ) , a portion of the ewes from the ASe and HSe groups was fed a restricted ( R ; 60 % of M ) diet .
	manualset3
233355	2	428144	15	NULL	NULL	0	NULL	pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	From day 50 to 132 of pregnancy ( tissue collection day ) , a portion of the ewes from the ASe and HSe groups was fed a restricted ( R ; 60 % of M ) diet .
	manualset3
233356	3	428144	15	NULL	NULL	0	NULL	tissue collection day	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	From day 50 to 132 of pregnancy ( tissue collection day ) , a portion of the ewes from the ASe and HSe groups was fed a restricted ( R ; 60 % of M ) diet .
	manualset3
233357	4	428144	15	NULL	NULL	0	NULL	portion	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	From day 50 to 132 of pregnancy ( tissue collection day ) , a portion of the ewes from the ASe and HSe groups was fed a restricted ( R ; 60 % of M ) diet .
	manualset3
233358	5	428144	15	NULL	NULL	0	NULL	 ewes	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	From day 50 to 132 of pregnancy ( tissue collection day ) , a portion of the ewes from the ASe and HSe groups was fed a restricted ( R ; 60 % of M ) diet .
	manualset3
233359	6	428144	15	NULL	NULL	0	NULL	ASe groups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	From day 50 to 132 of pregnancy ( tissue collection day ) , a portion of the ewes from the ASe and HSe groups was fed a restricted ( R ; 60 % of M ) diet .
	manualset3
233360	7	428144	15	NULL	NULL	0	NULL	HSe groups	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	From day 50 to 132 of pregnancy ( tissue collection day ) , a portion of the ewes from the ASe and HSe groups was fed a restricted ( R ; 60 % of M ) diet .
	manualset3
233361	8	428144	15	NULL	NULL	0	NULL	R ; 60 % of M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	From day 50 to 132 of pregnancy ( tissue collection day ) , a portion of the ewes from the ASe and HSe groups was fed a restricted ( R ; 60 % of M ) diet .
	manualset3
233362	9	428144	15	NULL	NULL	0	NULL	diet	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	From day 50 to 132 of pregnancy ( tissue collection day ) , a portion of the ewes from the ASe and HSe groups was fed a restricted ( R ; 60 % of M ) diet .
	manualset3
233363	1	428145	15	NULL	NULL	NULL	NULL	trial	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From each trial , common data elements were pooled to assess , principally , for correctness of thrombolysis decision-making .
	manualset3
233364	2	428145	15	NULL	NULL	0	NULL	data elements	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	From each trial , common data elements were pooled to assess , principally , for correctness of thrombolysis decision-making .
	manualset3
233365	3	428145	15	NULL	NULL	0	NULL	correctness	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	From each trial , common data elements were pooled to assess , principally , for correctness of thrombolysis decision-making .
	manualset3
233366	4	428145	15	NULL	NULL	0	NULL	thrombolysis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	From each trial , common data elements were pooled to assess , principally , for correctness of thrombolysis decision-making .
	manualset3
234739	5	428145	15	NULL	NULL	0	NULL	decision-making	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	From each trial , common data elements were pooled to assess , principally , for correctness of thrombolysis decision-making .
	manualset3
233367	1	428146	15	NULL	NULL	0	NULL	isotope experiments	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	From isotope experiments and whole-mount autoradiographs the tympanic mitotic activity appeared to be confined to an area close to the annulus typmpanicus .
	manualset3
233368	2	428146	15	NULL	NULL	0	NULL	whole-mount autoradiographs	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	From isotope experiments and whole-mount autoradiographs the tympanic mitotic activity appeared to be confined to an area close to the annulus typmpanicus .
	manualset3
233369	3	428146	15	NULL	NULL	NULL	NULL	tympanic mitotic activity	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From isotope experiments and whole-mount autoradiographs the tympanic mitotic activity appeared to be confined to an area close to the annulus typmpanicus .
	manualset3
233370	4	428146	15	NULL	NULL	0	NULL	area	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	From isotope experiments and whole-mount autoradiographs the tympanic mitotic activity appeared to be confined to an area close to the annulus typmpanicus .
	manualset3
233371	5	428146	15	NULL	NULL	0	NULL	annulus typmpanicus	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	From isotope experiments and whole-mount autoradiographs the tympanic mitotic activity appeared to be confined to an area close to the annulus typmpanicus .
	manualset3
233372	1	428147	15	NULL	NULL	0	NULL	experience	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	From our limited experience , it appears that Sialtx study is of value when CEA failed to indicate the presence of breast malignancy .
	manualset3
233373	2	428147	15	NULL	NULL	0	NULL	Sialtx study	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	From our limited experience , it appears that Sialtx study is of value when CEA failed to indicate the presence of breast malignancy .
	manualset3
233374	3	428147	15	NULL	NULL	0	NULL	value	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	From our limited experience , it appears that Sialtx study is of value when CEA failed to indicate the presence of breast malignancy .
	manualset3
233375	4	428147	15	NULL	NULL	0	NULL	CEA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	From our limited experience , it appears that Sialtx study is of value when CEA failed to indicate the presence of breast malignancy .
	manualset3
233376	5	428147	15	NULL	NULL	0	NULL	presence	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	From our limited experience , it appears that Sialtx study is of value when CEA failed to indicate the presence of breast malignancy .
	manualset3
233377	6	428147	15	NULL	NULL	0	NULL	breast malignancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	From our limited experience , it appears that Sialtx study is of value when CEA failed to indicate the presence of breast malignancy .
	manualset3
233378	1	428148	15	NULL	NULL	NULL	NULL	observations	MentalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From our observations we identified a panel of genes with cancer specific-epigenetic mediated aberrant expression including those with reported carcinogenic functions and members potentially mediating a positive epigenetic feedback loop .
	manualset3
233379	2	428148	15	NULL	NULL	0	NULL	panel of genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	From our observations we identified a panel of genes with cancer specific-epigenetic mediated aberrant expression including those with reported carcinogenic functions and members potentially mediating a positive epigenetic feedback loop .
	manualset3
233380	3	428148	15	NULL	NULL	0	NULL	cancer specific aberrant expression	MedicalDevice												NULL		0	NULL	NULL	NULL	NULL	NULL	From our observations we identified a panel of genes with cancer specific-epigenetic mediated aberrant expression including those with reported carcinogenic functions and members potentially mediating a positive epigenetic feedback loop .
	manualset3
233381	4	428148	15	NULL	NULL	0	NULL	epigenetic mediated aberrant expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	From our observations we identified a panel of genes with cancer specific-epigenetic mediated aberrant expression including those with reported carcinogenic functions and members potentially mediating a positive epigenetic feedback loop .
	manualset3
233382	5	428148	15	NULL	NULL	0	NULL	carcinogenic functions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	From our observations we identified a panel of genes with cancer specific-epigenetic mediated aberrant expression including those with reported carcinogenic functions and members potentially mediating a positive epigenetic feedback loop .
	manualset3
233383	6	428148	15	NULL	NULL	0	NULL	members	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	From our observations we identified a panel of genes with cancer specific-epigenetic mediated aberrant expression including those with reported carcinogenic functions and members potentially mediating a positive epigenetic feedback loop .
	manualset3
233384	7	428148	15	NULL	NULL	0	NULL	positive epigenetic feedback loop	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	From our observations we identified a panel of genes with cancer specific-epigenetic mediated aberrant expression including those with reported carcinogenic functions and members potentially mediating a positive epigenetic feedback loop .
	manualset3
233385	1	428149	15	NULL	NULL	NULL	NULL	specific features	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From specific features of radio occultation and other Voyager results , however , it is concluded that nitrogen does not condense on Titan and that Titan has neither global methane oceans nor a global cloud of liquid methane droplets .
	manualset3
233386	2	428149	15	NULL	NULL	NULL	NULL	radio occultation results	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From specific features of radio occultation and other Voyager results , however , it is concluded that nitrogen does not condense on Titan and that Titan has neither global methane oceans nor a global cloud of liquid methane droplets .
	manualset3
233387	3	428149	15	NULL	NULL	NULL	NULL	Voyager results	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From specific features of radio occultation and other Voyager results , however , it is concluded that nitrogen does not condense on Titan and that Titan has neither global methane oceans nor a global cloud of liquid methane droplets .
	manualset3
233388	4	428149	15	NULL	NULL	NULL	NULL	nitrogen	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From specific features of radio occultation and other Voyager results , however , it is concluded that nitrogen does not condense on Titan and that Titan has neither global methane oceans nor a global cloud of liquid methane droplets .
	manualset3
233389	5	428149	15	NULL	NULL	NULL	NULL	Titan	UnproperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From specific features of radio occultation and other Voyager results , however , it is concluded that nitrogen does not condense on Titan and that Titan has neither global methane oceans nor a global cloud of liquid methane droplets .
	manualset3
233390	6	428149	15	NULL	NULL	0	NULL	Titan	UnproperNamedGeographicalLocation												NULL		0	NULL	NULL	NULL	NULL	NULL	From specific features of radio occultation and other Voyager results , however , it is concluded that nitrogen does not condense on Titan and that Titan has neither global methane oceans nor a global cloud of liquid methane droplets .
	manualset3
233391	7	428149	15	NULL	NULL	0	NULL	methane oceans	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	From specific features of radio occultation and other Voyager results , however , it is concluded that nitrogen does not condense on Titan and that Titan has neither global methane oceans nor a global cloud of liquid methane droplets .
	manualset3
233392	8	428149	15	NULL	NULL	0	NULL	cloud	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	From specific features of radio occultation and other Voyager results , however , it is concluded that nitrogen does not condense on Titan and that Titan has neither global methane oceans nor a global cloud of liquid methane droplets .
	manualset3
233393	9	428149	15	NULL	NULL	0	NULL	methane droplets	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	From specific features of radio occultation and other Voyager results , however , it is concluded that nitrogen does not condense on Titan and that Titan has neither global methane oceans nor a global cloud of liquid methane droplets .
	manualset3
233853	1	428150	15	NULL	NULL	0	NULL	study	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	From study of the late-term results of treatment of a large group of patients ( children , adults with a thymus ) the main causes of unsuccessful surgical treatment of generalized myasthenia were identified and the concrete means of improving the results of treatment were planned .
	manualset3
233854	2	428150	15	NULL	NULL	0	NULL	results	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	From study of the late-term results of treatment of a large group of patients ( children , adults with a thymus ) the main causes of unsuccessful surgical treatment of generalized myasthenia were identified and the concrete means of improving the results of treatment were planned .
	manualset3
233855	3	428150	15	NULL	NULL	0	NULL	treatment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	From study of the late-term results of treatment of a large group of patients ( children , adults with a thymus ) the main causes of unsuccessful surgical treatment of generalized myasthenia were identified and the concrete means of improving the results of treatment were planned .
	manualset3
233856	4	428150	15	NULL	NULL	0	NULL	group of patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	From study of the late-term results of treatment of a large group of patients ( children , adults with a thymus ) the main causes of unsuccessful surgical treatment of generalized myasthenia were identified and the concrete means of improving the results of treatment were planned .
	manualset3
233857	5	428150	15	NULL	NULL	0	NULL	children with a thymus	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	From study of the late-term results of treatment of a large group of patients ( children , adults with a thymus ) the main causes of unsuccessful surgical treatment of generalized myasthenia were identified and the concrete means of improving the results of treatment were planned .
	manualset3
233858	6	428150	15	NULL	NULL	0	NULL	adults with a thymus	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	From study of the late-term results of treatment of a large group of patients ( children , adults with a thymus ) the main causes of unsuccessful surgical treatment of generalized myasthenia were identified and the concrete means of improving the results of treatment were planned .
	manualset3
233861	7	428150	15	NULL	NULL	0	NULL	causes	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	From study of the late-term results of treatment of a large group of patients ( children , adults with a thymus ) the main causes of unsuccessful surgical treatment of generalized myasthenia were identified and the concrete means of improving the results of treatment were planned .
	manualset3
233864	8	428150	15	NULL	NULL	0	NULL	surgical treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	From study of the late-term results of treatment of a large group of patients ( children , adults with a thymus ) the main causes of unsuccessful surgical treatment of generalized myasthenia were identified and the concrete means of improving the results of treatment were planned .
	manualset3
233867	9	428150	15	NULL	NULL	0	NULL	myasthenia	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	From study of the late-term results of treatment of a large group of patients ( children , adults with a thymus ) the main causes of unsuccessful surgical treatment of generalized myasthenia were identified and the concrete means of improving the results of treatment were planned .
	manualset3
233868	10	428150	15	NULL	NULL	0	NULL	means	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	From study of the late-term results of treatment of a large group of patients ( children , adults with a thymus ) the main causes of unsuccessful surgical treatment of generalized myasthenia were identified and the concrete means of improving the results of treatment were planned .
	manualset3
233869	11	428150	15	NULL	NULL	0	NULL	results 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	From study of the late-term results of treatment of a large group of patients ( children , adults with a thymus ) the main causes of unsuccessful surgical treatment of generalized myasthenia were identified and the concrete means of improving the results of treatment were planned .
	manualset3
233870	12	428150	15	NULL	NULL	0	NULL	treatment 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	From study of the late-term results of treatment of a large group of patients ( children , adults with a thymus ) the main causes of unsuccessful surgical treatment of generalized myasthenia were identified and the concrete means of improving the results of treatment were planned .
	manualset3
233876	1	428151	15	NULL	NULL	0	NULL	AIMD simulation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	From the AIMD simulation , the distribution of the head-on rings of acetic acid is revealed and shows that the favorable structures tend to be the acetic acid hydrates rather than the HAc cyclic dimer .
	manualset3
233877	2	428151	15	NULL	NULL	0	NULL	distribution	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	From the AIMD simulation , the distribution of the head-on rings of acetic acid is revealed and shows that the favorable structures tend to be the acetic acid hydrates rather than the HAc cyclic dimer .
	manualset3
233878	3	428151	15	NULL	NULL	NULL	NULL	head-on rings	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From the AIMD simulation , the distribution of the head-on rings of acetic acid is revealed and shows that the favorable structures tend to be the acetic acid hydrates rather than the HAc cyclic dimer .
	manualset3
233879	4	428151	15	NULL	NULL	0	NULL	acetic acid	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	From the AIMD simulation , the distribution of the head-on rings of acetic acid is revealed and shows that the favorable structures tend to be the acetic acid hydrates rather than the HAc cyclic dimer .
	manualset3
233880	5	428151	15	NULL	NULL	NULL	NULL	structures	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From the AIMD simulation , the distribution of the head-on rings of acetic acid is revealed and shows that the favorable structures tend to be the acetic acid hydrates rather than the HAc cyclic dimer .
	manualset3
233881	6	428151	15	NULL	NULL	0	NULL	acetic acid hydrates	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	From the AIMD simulation , the distribution of the head-on rings of acetic acid is revealed and shows that the favorable structures tend to be the acetic acid hydrates rather than the HAc cyclic dimer .
	manualset3
233882	7	428151	15	NULL	NULL	0	NULL	HAc cyclic dimer	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	From the AIMD simulation , the distribution of the head-on rings of acetic acid is revealed and shows that the favorable structures tend to be the acetic acid hydrates rather than the HAc cyclic dimer .
	manualset3
233896	1	428152	15	NULL	NULL	0	NULL	facts	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	From the above facts , it was assumed that the inhibitory substance of GAP-Dehyd in urine of diabetics was a new acidic compound of low molecular weight containing an amino residue in the molecule .
	manualset3
233904	2	428152	15	NULL	NULL	NULL	NULL	substance	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From the above facts , it was assumed that the inhibitory substance of GAP-Dehyd in urine of diabetics was a new acidic compound of low molecular weight containing an amino residue in the molecule .
	manualset3
233910	3	428152	15	NULL	NULL	0	NULL	GAP-Dehyd	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	From the above facts , it was assumed that the inhibitory substance of GAP-Dehyd in urine of diabetics was a new acidic compound of low molecular weight containing an amino residue in the molecule .
	manualset3
233914	4	428152	15	NULL	NULL	0	NULL	urine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	From the above facts , it was assumed that the inhibitory substance of GAP-Dehyd in urine of diabetics was a new acidic compound of low molecular weight containing an amino residue in the molecule .
	manualset3
233915	5	428152	15	NULL	NULL	0	NULL	diabetics	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	From the above facts , it was assumed that the inhibitory substance of GAP-Dehyd in urine of diabetics was a new acidic compound of low molecular weight containing an amino residue in the molecule .
	manualset3
233916	6	428152	15	NULL	NULL	0	NULL	acidic compound	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	From the above facts , it was assumed that the inhibitory substance of GAP-Dehyd in urine of diabetics was a new acidic compound of low molecular weight containing an amino residue in the molecule .
	manualset3
233918	7	428152	15	NULL	NULL	0	NULL	molecular weight	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	From the above facts , it was assumed that the inhibitory substance of GAP-Dehyd in urine of diabetics was a new acidic compound of low molecular weight containing an amino residue in the molecule .
	manualset3
233929	8	428152	15	NULL	NULL	NULL	NULL	amino residue	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From the above facts , it was assumed that the inhibitory substance of GAP-Dehyd in urine of diabetics was a new acidic compound of low molecular weight containing an amino residue in the molecule .
	manualset3
233930	9	428152	15	NULL	NULL	0	NULL	 molecule 	Molecule												NULL		0	NULL	NULL	NULL	NULL	NULL	From the above facts , it was assumed that the inhibitory substance of GAP-Dehyd in urine of diabetics was a new acidic compound of low molecular weight containing an amino residue in the molecule .
	manualset3
233931	1	428153	15	NULL	NULL	0	NULL	Retroactive evaluation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Retroactive evaluation of perioperative staging and surgical decision making for patients with pancreatic cancer ) .
	manualset3
233932	2	428153	15	NULL	NULL	0	NULL	perioperative staging	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Retroactive evaluation of perioperative staging and surgical decision making for patients with pancreatic cancer ) .
	manualset3
233933	3	428153	15	NULL	NULL	0	NULL	surgical decision making	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Retroactive evaluation of perioperative staging and surgical decision making for patients with pancreatic cancer ) .
	manualset3
233934	4	428153	15	NULL	NULL	0	NULL	patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Retroactive evaluation of perioperative staging and surgical decision making for patients with pancreatic cancer ) .
	manualset3
233935	5	428153	15	NULL	NULL	0	NULL	pancreatic cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	( Retroactive evaluation of perioperative staging and surgical decision making for patients with pancreatic cancer ) .
	manualset3
233936	1	428154	15	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	From the analysis of LVG , the rapid filling fraction ( RFF ) , and the atrial filling fraction ( AFF ) were obtained .
	manualset3
233937	2	428154	15	NULL	NULL	0	NULL	LVG	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	From the analysis of LVG , the rapid filling fraction ( RFF ) , and the atrial filling fraction ( AFF ) were obtained .
	manualset3
233938	3	428154	15	NULL	NULL	0	NULL	rapid filling fraction ( RFF )	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	From the analysis of LVG , the rapid filling fraction ( RFF ) , and the atrial filling fraction ( AFF ) were obtained .
	manualset3
233939	4	428154	15	NULL	NULL	0	NULL	atrial filling fraction ( AFF ) 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	From the analysis of LVG , the rapid filling fraction ( RFF ) , and the atrial filling fraction ( AFF ) were obtained .
	manualset3
233940	1	428155	15	NULL	NULL	0	NULL	least charged state	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	From the least charged state , the O2 can react with CO adsorbed at the edge sites of the Au particles leading to the formation of CO2 with very low ( approximately 0.15 eV ) energy barriers .
	manualset3
233941	2	428155	15	NULL	NULL	0	NULL	O2	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	From the least charged state , the O2 can react with CO adsorbed at the edge sites of the Au particles leading to the formation of CO2 with very low ( approximately 0.15 eV ) energy barriers .
	manualset3
233942	3	428155	15	NULL	NULL	0	NULL	CO	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	From the least charged state , the O2 can react with CO adsorbed at the edge sites of the Au particles leading to the formation of CO2 with very low ( approximately 0.15 eV ) energy barriers .
	manualset3
233943	4	428155	15	NULL	NULL	0	NULL	edge sites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	From the least charged state , the O2 can react with CO adsorbed at the edge sites of the Au particles leading to the formation of CO2 with very low ( approximately 0.15 eV ) energy barriers .
	manualset3
233944	5	428155	15	NULL	NULL	0	NULL	Au particles 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	From the least charged state , the O2 can react with CO adsorbed at the edge sites of the Au particles leading to the formation of CO2 with very low ( approximately 0.15 eV ) energy barriers .
	manualset3
233945	6	428155	15	NULL	NULL	0	NULL	formation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	From the least charged state , the O2 can react with CO adsorbed at the edge sites of the Au particles leading to the formation of CO2 with very low ( approximately 0.15 eV ) energy barriers .
	manualset3
233946	7	428155	15	NULL	NULL	0	NULL	CO2 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	From the least charged state , the O2 can react with CO adsorbed at the edge sites of the Au particles leading to the formation of CO2 with very low ( approximately 0.15 eV ) energy barriers .
	manualset3
233947	8	428155	15	NULL	NULL	0	NULL	0.15 eV	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	From the least charged state , the O2 can react with CO adsorbed at the edge sites of the Au particles leading to the formation of CO2 with very low ( approximately 0.15 eV ) energy barriers .
	manualset3
233948	9	428155	15	NULL	NULL	0	NULL	energy barriers	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	From the least charged state , the O2 can react with CO adsorbed at the edge sites of the Au particles leading to the formation of CO2 with very low ( approximately 0.15 eV ) energy barriers .
	manualset3
233949	1	428156	15	NULL	NULL	NULL	NULL	study 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From the present study it is evident that severe RA may be accompanied by AN and the consequences need to be elucidated .
	manualset3
233950	2	428156	15	NULL	NULL	0	NULL	RA	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	From the present study it is evident that severe RA may be accompanied by AN and the consequences need to be elucidated .
	manualset3
233951	3	428156	15	NULL	NULL	0	NULL	AN	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	From the present study it is evident that severe RA may be accompanied by AN and the consequences need to be elucidated .
	manualset3
233952	4	428156	15	NULL	NULL	NULL	NULL	consequences	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From the present study it is evident that severe RA may be accompanied by AN and the consequences need to be elucidated .
	manualset3
233953	1	428157	15	NULL	NULL	0	NULL	reported case	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	From the reported case , the authors discuss the possible part of mineral oil as pleural carcinogenic factor ( mesothelioma ) .
	manualset3
233954	2	428157	15	NULL	NULL	0	NULL	authors 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	From the reported case , the authors discuss the possible part of mineral oil as pleural carcinogenic factor ( mesothelioma ) .
	manualset3
233955	3	428157	15	NULL	NULL	0	NULL	part 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	From the reported case , the authors discuss the possible part of mineral oil as pleural carcinogenic factor ( mesothelioma ) .
	manualset3
233956	4	428157	15	NULL	NULL	0	NULL	mineral oil	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	From the reported case , the authors discuss the possible part of mineral oil as pleural carcinogenic factor ( mesothelioma ) .
	manualset3
233957	5	428157	15	NULL	NULL	0	NULL	pleural carcinogenic factor	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	From the reported case , the authors discuss the possible part of mineral oil as pleural carcinogenic factor ( mesothelioma ) .
	manualset3
233958	6	428157	15	NULL	NULL	0	NULL	mesothelioma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	From the reported case , the authors discuss the possible part of mineral oil as pleural carcinogenic factor ( mesothelioma ) .
	manualset3
233959	1	428158	15	NULL	NULL	0	NULL	results	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	From the results , it appears that the catalytic effect of biocatalyst of the dehydroascorbic reduction by thiols has no direct relation with the redox properties .
	manualset3
233960	2	428158	15	NULL	NULL	NULL	NULL	catalytic effect	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From the results , it appears that the catalytic effect of biocatalyst of the dehydroascorbic reduction by thiols has no direct relation with the redox properties .
	manualset3
233961	4	428158	15	NULL	NULL	NULL	NULL	dehydroascorbic reduction	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From the results , it appears that the catalytic effect of biocatalyst of the dehydroascorbic reduction by thiols has no direct relation with the redox properties .
	manualset3
233962	5	428158	15	NULL	NULL	NULL	NULL	thiols 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From the results , it appears that the catalytic effect of biocatalyst of the dehydroascorbic reduction by thiols has no direct relation with the redox properties .
	manualset3
233963	6	428158	15	NULL	NULL	NULL	NULL	direct relation	Relationship												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From the results , it appears that the catalytic effect of biocatalyst of the dehydroascorbic reduction by thiols has no direct relation with the redox properties .
	manualset3
233964	7	428158	15	NULL	NULL	NULL	NULL	redox properties	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From the results , it appears that the catalytic effect of biocatalyst of the dehydroascorbic reduction by thiols has no direct relation with the redox properties .
	manualset3
235751	3	428158	15	NULL	NULL	0	NULL	biocatalyst 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	From the results , it appears that the catalytic effect of biocatalyst of the dehydroascorbic reduction by thiols has no direct relation with the redox properties .
	manualset3
233965	1	428159	15	NULL	NULL	0	NULL	results	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	From the results reported for the flavan-3-ol family , their anti-amyloidogenic effects against whole peptides ( 1-40 and 1-42 ) could involve several binding sites .
	manualset3
233966	2	428159	15	NULL	NULL	0	NULL	flavan-3-ol family	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	From the results reported for the flavan-3-ol family , their anti-amyloidogenic effects against whole peptides ( 1-40 and 1-42 ) could involve several binding sites .
	manualset3
233967	3	428159	15	NULL	NULL	0	NULL	anti-amyloidogenic effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	From the results reported for the flavan-3-ol family , their anti-amyloidogenic effects against whole peptides ( 1-40 and 1-42 ) could involve several binding sites .
	manualset3
233968	4	428159	15	NULL	NULL	0	NULL	peptides ( 1-40)	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	From the results reported for the flavan-3-ol family , their anti-amyloidogenic effects against whole peptides ( 1-40 and 1-42 ) could involve several binding sites .
	manualset3
233969	5	428159	15	NULL	NULL	0	NULL	peptides (1-42 )	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	From the results reported for the flavan-3-ol family , their anti-amyloidogenic effects against whole peptides ( 1-40 and 1-42 ) could involve several binding sites .
	manualset3
233970	6	428159	15	NULL	NULL	0	NULL	binding sites	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	From the results reported for the flavan-3-ol family , their anti-amyloidogenic effects against whole peptides ( 1-40 and 1-42 ) could involve several binding sites .
	manualset3
233971	1	428160	15	NULL	NULL	0	NULL	standpoint	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	From the standpoint of self-preservation of the organism the above-named changes can be regarded as quite expedient since they minimize the action of adverse factors of the labor process .
	manualset3
233972	2	428160	15	NULL	NULL	0	NULL	self-preservation 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	From the standpoint of self-preservation of the organism the above-named changes can be regarded as quite expedient since they minimize the action of adverse factors of the labor process .
	manualset3
233973	3	428160	15	NULL	NULL	0	NULL	organism	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	From the standpoint of self-preservation of the organism the above-named changes can be regarded as quite expedient since they minimize the action of adverse factors of the labor process .
	manualset3
233974	4	428160	15	NULL	NULL	0	NULL	named changes 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	From the standpoint of self-preservation of the organism the above-named changes can be regarded as quite expedient since they minimize the action of adverse factors of the labor process .
	manualset3
233975	5	428160	15	NULL	NULL	0	NULL	action	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	From the standpoint of self-preservation of the organism the above-named changes can be regarded as quite expedient since they minimize the action of adverse factors of the labor process .
	manualset3
233976	6	428160	15	NULL	NULL	0	NULL	adverse factors	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	From the standpoint of self-preservation of the organism the above-named changes can be regarded as quite expedient since they minimize the action of adverse factors of the labor process .
	manualset3
233977	7	428160	15	NULL	NULL	0	NULL	labor process	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	From the standpoint of self-preservation of the organism the above-named changes can be regarded as quite expedient since they minimize the action of adverse factors of the labor process .
	manualset3
233978	1	428161	15	NULL	NULL	0	NULL	whole plants 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	From the whole plants of Corydalis tashiroi Makino a new quaternary protoberberinium base dehydrodiscretamine chloride was isolated along with four known quaternary alkaloids by the application of droplet countercurrent chromatography ( DCCC ) .
	manualset3
233979	2	428161	15	NULL	NULL	0	NULL	Corydalis tashiroi Makino	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	From the whole plants of Corydalis tashiroi Makino a new quaternary protoberberinium base dehydrodiscretamine chloride was isolated along with four known quaternary alkaloids by the application of droplet countercurrent chromatography ( DCCC ) .
	manualset3
233980	3	428161	15	NULL	NULL	0	NULL	quaternary protoberberinium base dehydrodiscretamine chloride 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	From the whole plants of Corydalis tashiroi Makino a new quaternary protoberberinium base dehydrodiscretamine chloride was isolated along with four known quaternary alkaloids by the application of droplet countercurrent chromatography ( DCCC ) .
	manualset3
233981	4	428161	15	NULL	NULL	0	NULL	four 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	From the whole plants of Corydalis tashiroi Makino a new quaternary protoberberinium base dehydrodiscretamine chloride was isolated along with four known quaternary alkaloids by the application of droplet countercurrent chromatography ( DCCC ) .
	manualset3
233982	5	428161	15	NULL	NULL	0	NULL	quaternary alkaloids	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	From the whole plants of Corydalis tashiroi Makino a new quaternary protoberberinium base dehydrodiscretamine chloride was isolated along with four known quaternary alkaloids by the application of droplet countercurrent chromatography ( DCCC ) .
	manualset3
233984	6	428161	15	NULL	NULL	0	NULL	application	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	From the whole plants of Corydalis tashiroi Makino a new quaternary protoberberinium base dehydrodiscretamine chloride was isolated along with four known quaternary alkaloids by the application of droplet countercurrent chromatography ( DCCC ) .
	manualset3
233985	7	428161	15	NULL	NULL	0	NULL	droplet countercurrent chromatography ( DCCC )	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	From the whole plants of Corydalis tashiroi Makino a new quaternary protoberberinium base dehydrodiscretamine chloride was isolated along with four known quaternary alkaloids by the application of droplet countercurrent chromatography ( DCCC ) .
	manualset3
233986	1	428162	15	NULL	NULL	0	NULL	 802 nurses 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	From these , a total of 802 nurses ( 71 % ) reported blood and body fluid exposure incidents during 2003-2005 and this group was used for analysis .
	manualset3
233987	2	428162	15	NULL	NULL	0	NULL	71 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	From these , a total of 802 nurses ( 71 % ) reported blood and body fluid exposure incidents during 2003-2005 and this group was used for analysis .
	manualset3
233988	3	428162	15	NULL	NULL	NULL	NULL	blood exposure	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From these , a total of 802 nurses ( 71 % ) reported blood and body fluid exposure incidents during 2003-2005 and this group was used for analysis .
	manualset3
233989	4	428162	15	NULL	NULL	0	NULL	body fluid exposure	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	From these , a total of 802 nurses ( 71 % ) reported blood and body fluid exposure incidents during 2003-2005 and this group was used for analysis .
	manualset3
233990	5	428162	15	NULL	NULL	0	NULL	incidents	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	From these , a total of 802 nurses ( 71 % ) reported blood and body fluid exposure incidents during 2003-2005 and this group was used for analysis .
	manualset3
233991	6	428162	15	NULL	NULL	0	NULL	2003-2005	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	From these , a total of 802 nurses ( 71 % ) reported blood and body fluid exposure incidents during 2003-2005 and this group was used for analysis .
	manualset3
233992	7	428162	15	NULL	NULL	0	NULL	group	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	From these , a total of 802 nurses ( 71 % ) reported blood and body fluid exposure incidents during 2003-2005 and this group was used for analysis .
	manualset3
233993	8	428162	15	NULL	NULL	0	NULL	analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	From these , a total of 802 nurses ( 71 % ) reported blood and body fluid exposure incidents during 2003-2005 and this group was used for analysis .
	manualset3
233994	1	428163	15	NULL	NULL	NULL	NULL	studies 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From these and other studies of Golgi membrane proteins , we now understand that a variety of retention mechanisms are employed , the majority of which involve the dynamic process of iterative rounds of retrograde and anterograde transport .
	manualset3
233995	2	428163	15	NULL	NULL	NULL	NULL	Golgi membrane proteins 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From these and other studies of Golgi membrane proteins , we now understand that a variety of retention mechanisms are employed , the majority of which involve the dynamic process of iterative rounds of retrograde and anterograde transport .
	manualset3
233996	3	428163	15	NULL	NULL	0	NULL	retention mechanisms 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	From these and other studies of Golgi membrane proteins , we now understand that a variety of retention mechanisms are employed , the majority of which involve the dynamic process of iterative rounds of retrograde and anterograde transport .
	manualset3
233997	4	428163	15	NULL	NULL	0	NULL	majority	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	From these and other studies of Golgi membrane proteins , we now understand that a variety of retention mechanisms are employed , the majority of which involve the dynamic process of iterative rounds of retrograde and anterograde transport .
	manualset3
233999	5	428163	15	NULL	NULL	0	NULL	dynamic process	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	From these and other studies of Golgi membrane proteins , we now understand that a variety of retention mechanisms are employed , the majority of which involve the dynamic process of iterative rounds of retrograde and anterograde transport .
	manualset3
234000	6	428163	15	NULL	NULL	0	NULL	 retrograde transport	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	From these and other studies of Golgi membrane proteins , we now understand that a variety of retention mechanisms are employed , the majority of which involve the dynamic process of iterative rounds of retrograde and anterograde transport .
	manualset3
234001	7	428163	15	NULL	NULL	0	NULL	anterograde transport	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	From these and other studies of Golgi membrane proteins , we now understand that a variety of retention mechanisms are employed , the majority of which involve the dynamic process of iterative rounds of retrograde and anterograde transport .
	manualset3
234006	1	428164	15	NULL	NULL	0	NULL	results	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	From these results , the amino acid sequence of the site cleaved by trypsin was extended to cover the C termini ( present in VP8 ) .
	manualset3
234011	2	428164	15	NULL	NULL	0	NULL	 amino acid sequence	AminoAcidPeptide												NULL		0	NULL	NULL	NULL	NULL	NULL	From these results , the amino acid sequence of the site cleaved by trypsin was extended to cover the C termini ( present in VP8 ) .
	manualset3
234012	3	428164	15	NULL	NULL	0	NULL	site	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	From these results , the amino acid sequence of the site cleaved by trypsin was extended to cover the C termini ( present in VP8 ) .
	manualset3
234013	4	428164	15	NULL	NULL	0	NULL	trypsin	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	From these results , the amino acid sequence of the site cleaved by trypsin was extended to cover the C termini ( present in VP8 ) .
	manualset3
234014	5	428164	15	NULL	NULL	0	NULL	C termini 	PartOfProtein												NULL		0	NULL	NULL	NULL	NULL	NULL	From these results , the amino acid sequence of the site cleaved by trypsin was extended to cover the C termini ( present in VP8 ) .
	manualset3
234015	6	428164	15	NULL	NULL	NULL	NULL	VP8 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From these results , the amino acid sequence of the site cleaved by trypsin was extended to cover the C termini ( present in VP8 ) .
	manualset3
234016	1	428165	15	NULL	NULL	NULL	NULL	studies 	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From these studies a drug evaluation protocol was developed using 150 NaL3 as the infectious dose and then evaluating the anthelminthic effects of the drugs albendazole , tribendimidine , and pyrantel pamoate on days 21-28 post-infection .
	manualset3
234017	2	428165	15	NULL	NULL	0	NULL	drug evaluation protocol 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	From these studies a drug evaluation protocol was developed using 150 NaL3 as the infectious dose and then evaluating the anthelminthic effects of the drugs albendazole , tribendimidine , and pyrantel pamoate on days 21-28 post-infection .
	manualset3
234018	3	428165	15	NULL	NULL	0	NULL	150 NaL3	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	From these studies a drug evaluation protocol was developed using 150 NaL3 as the infectious dose and then evaluating the anthelminthic effects of the drugs albendazole , tribendimidine , and pyrantel pamoate on days 21-28 post-infection .
	manualset3
234022	4	428165	15	NULL	NULL	0	NULL	infectious dose 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	From these studies a drug evaluation protocol was developed using 150 NaL3 as the infectious dose and then evaluating the anthelminthic effects of the drugs albendazole , tribendimidine , and pyrantel pamoate on days 21-28 post-infection .
	manualset3
234025	5	428165	15	NULL	NULL	0	NULL	anthelminthic effects	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	From these studies a drug evaluation protocol was developed using 150 NaL3 as the infectious dose and then evaluating the anthelminthic effects of the drugs albendazole , tribendimidine , and pyrantel pamoate on days 21-28 post-infection .
	manualset3
234027	6	428165	15	NULL	NULL	0	NULL	drugs	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	From these studies a drug evaluation protocol was developed using 150 NaL3 as the infectious dose and then evaluating the anthelminthic effects of the drugs albendazole , tribendimidine , and pyrantel pamoate on days 21-28 post-infection .
	manualset3
234028	7	428165	15	NULL	NULL	0	NULL	albendazole	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	From these studies a drug evaluation protocol was developed using 150 NaL3 as the infectious dose and then evaluating the anthelminthic effects of the drugs albendazole , tribendimidine , and pyrantel pamoate on days 21-28 post-infection .
	manualset3
234029	8	428165	15	NULL	NULL	0	NULL	tribendimidine	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	From these studies a drug evaluation protocol was developed using 150 NaL3 as the infectious dose and then evaluating the anthelminthic effects of the drugs albendazole , tribendimidine , and pyrantel pamoate on days 21-28 post-infection .
	manualset3
234030	9	428165	15	NULL	NULL	0	NULL	pyrantel pamoate	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	From these studies a drug evaluation protocol was developed using 150 NaL3 as the infectious dose and then evaluating the anthelminthic effects of the drugs albendazole , tribendimidine , and pyrantel pamoate on days 21-28 post-infection .
	manualset3
234033	10	428165	15	NULL	NULL	0	NULL	days 21-28 post-infection	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	From these studies a drug evaluation protocol was developed using 150 NaL3 as the infectious dose and then evaluating the anthelminthic effects of the drugs albendazole , tribendimidine , and pyrantel pamoate on days 21-28 post-infection .
	manualset3
234039	1	428166	15	NULL	NULL	NULL	NULL	trees	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From these trees , the Agrocybe coding introns argue for recent lateral transfers , i.e. , occurring after the separation of the two Agrocybe species , involving phylogenetically distant fungi such as members of the Ascomycota phylum ( for iAch1 and iAae2 ) and , for the first time to our knowledge , a member of the Chytridiomycota phylum ( for iAae1 ) .
	manualset3
234040	2	428166	15	NULL	NULL	NULL	NULL	Agrocybe coding introns	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From these trees , the Agrocybe coding introns argue for recent lateral transfers , i.e. , occurring after the separation of the two Agrocybe species , involving phylogenetically distant fungi such as members of the Ascomycota phylum ( for iAch1 and iAae2 ) and , for the first time to our knowledge , a member of the Chytridiomycota phylum ( for iAae1 ) .
	manualset3
234049	3	428166	15	NULL	NULL	0	NULL	lateral transfers 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	From these trees , the Agrocybe coding introns argue for recent lateral transfers , i.e. , occurring after the separation of the two Agrocybe species , involving phylogenetically distant fungi such as members of the Ascomycota phylum ( for iAch1 and iAae2 ) and , for the first time to our knowledge , a member of the Chytridiomycota phylum ( for iAae1 ) .
	manualset3
234051	4	428166	15	NULL	NULL	0	NULL	separation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	From these trees , the Agrocybe coding introns argue for recent lateral transfers , i.e. , occurring after the separation of the two Agrocybe species , involving phylogenetically distant fungi such as members of the Ascomycota phylum ( for iAch1 and iAae2 ) and , for the first time to our knowledge , a member of the Chytridiomycota phylum ( for iAae1 ) .
	manualset3
234052	5	428166	15	NULL	NULL	0	NULL	two Agrocybe species	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	From these trees , the Agrocybe coding introns argue for recent lateral transfers , i.e. , occurring after the separation of the two Agrocybe species , involving phylogenetically distant fungi such as members of the Ascomycota phylum ( for iAch1 and iAae2 ) and , for the first time to our knowledge , a member of the Chytridiomycota phylum ( for iAae1 ) .
	manualset3
234053	6	428166	15	NULL	NULL	0	NULL	phylogenetically distant fungi 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	From these trees , the Agrocybe coding introns argue for recent lateral transfers , i.e. , occurring after the separation of the two Agrocybe species , involving phylogenetically distant fungi such as members of the Ascomycota phylum ( for iAch1 and iAae2 ) and , for the first time to our knowledge , a member of the Chytridiomycota phylum ( for iAae1 ) .
	manualset3
234054	7	428166	15	NULL	NULL	0	NULL	members	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	From these trees , the Agrocybe coding introns argue for recent lateral transfers , i.e. , occurring after the separation of the two Agrocybe species , involving phylogenetically distant fungi such as members of the Ascomycota phylum ( for iAch1 and iAae2 ) and , for the first time to our knowledge , a member of the Chytridiomycota phylum ( for iAae1 ) .
	manualset3
234061	8	428166	15	NULL	NULL	0	NULL	 Ascomycota phylum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	From these trees , the Agrocybe coding introns argue for recent lateral transfers , i.e. , occurring after the separation of the two Agrocybe species , involving phylogenetically distant fungi such as members of the Ascomycota phylum ( for iAch1 and iAae2 ) and , for the first time to our knowledge , a member of the Chytridiomycota phylum ( for iAae1 ) .
	manualset3
234063	9	428166	15	NULL	NULL	NULL	NULL	iAch1	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From these trees , the Agrocybe coding introns argue for recent lateral transfers , i.e. , occurring after the separation of the two Agrocybe species , involving phylogenetically distant fungi such as members of the Ascomycota phylum ( for iAch1 and iAae2 ) and , for the first time to our knowledge , a member of the Chytridiomycota phylum ( for iAae1 ) .
	manualset3
234065	10	428166	15	NULL	NULL	NULL	NULL	iAae2	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From these trees , the Agrocybe coding introns argue for recent lateral transfers , i.e. , occurring after the separation of the two Agrocybe species , involving phylogenetically distant fungi such as members of the Ascomycota phylum ( for iAch1 and iAae2 ) and , for the first time to our knowledge , a member of the Chytridiomycota phylum ( for iAae1 ) .
	manualset3
234069	11	428166	15	NULL	NULL	0	NULL	first time	TimePoint												NULL		0	NULL	NULL	NULL	NULL	NULL	From these trees , the Agrocybe coding introns argue for recent lateral transfers , i.e. , occurring after the separation of the two Agrocybe species , involving phylogenetically distant fungi such as members of the Ascomycota phylum ( for iAch1 and iAae2 ) and , for the first time to our knowledge , a member of the Chytridiomycota phylum ( for iAae1 ) .
	manualset3
234071	12	428166	15	NULL	NULL	0	NULL	knowledge	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	From these trees , the Agrocybe coding introns argue for recent lateral transfers , i.e. , occurring after the separation of the two Agrocybe species , involving phylogenetically distant fungi such as members of the Ascomycota phylum ( for iAch1 and iAae2 ) and , for the first time to our knowledge , a member of the Chytridiomycota phylum ( for iAae1 ) .
	manualset3
234073	13	428166	15	NULL	NULL	0	NULL	member	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	From these trees , the Agrocybe coding introns argue for recent lateral transfers , i.e. , occurring after the separation of the two Agrocybe species , involving phylogenetically distant fungi such as members of the Ascomycota phylum ( for iAch1 and iAae2 ) and , for the first time to our knowledge , a member of the Chytridiomycota phylum ( for iAae1 ) .
	manualset3
234075	14	428166	15	NULL	NULL	0	NULL	Chytridiomycota phylum	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	From these trees , the Agrocybe coding introns argue for recent lateral transfers , i.e. , occurring after the separation of the two Agrocybe species , involving phylogenetically distant fungi such as members of the Ascomycota phylum ( for iAch1 and iAae2 ) and , for the first time to our knowledge , a member of the Chytridiomycota phylum ( for iAae1 ) .
	manualset3
234078	15	428166	15	NULL	NULL	NULL	NULL	iAae1 	NucleicAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From these trees , the Agrocybe coding introns argue for recent lateral transfers , i.e. , occurring after the separation of the two Agrocybe species , involving phylogenetically distant fungi such as members of the Ascomycota phylum ( for iAch1 and iAae2 ) and , for the first time to our knowledge , a member of the Chytridiomycota phylum ( for iAae1 ) .
	manualset3
234090	1	428167	15	NULL	NULL	0	NULL	two curves	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	From these two curves , it appeared that L-phenylalaninol may competitively inhibit the intestinal transport of L-phenylalanine .
	manualset3
234092	2	428167	15	NULL	NULL	0	NULL	L-phenylalaninol 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	From these two curves , it appeared that L-phenylalaninol may competitively inhibit the intestinal transport of L-phenylalanine .
	manualset3
234093	3	428167	15	NULL	NULL	0	NULL	intestinal transport	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	From these two curves , it appeared that L-phenylalaninol may competitively inhibit the intestinal transport of L-phenylalanine .
	manualset3
234094	4	428167	15	NULL	NULL	0	NULL	L-phenylalanine	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	From these two curves , it appeared that L-phenylalaninol may competitively inhibit the intestinal transport of L-phenylalanine .
	manualset3
234101	1	428168	15	NULL	NULL	0	NULL	discovery	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	From this discovery , we propose that LINE ORF1ps play a general role in LINE integration by forming a complex with LINE RNA and rearranging its conformation .
	manualset3
234116	2	428168	15	NULL	NULL	0	NULL	LINE ORF1ps	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	From this discovery , we propose that LINE ORF1ps play a general role in LINE integration by forming a complex with LINE RNA and rearranging its conformation .
	manualset3
234117	3	428168	15	NULL	NULL	NULL	NULL	role	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From this discovery , we propose that LINE ORF1ps play a general role in LINE integration by forming a complex with LINE RNA and rearranging its conformation .
	manualset3
234121	4	428168	15	NULL	NULL	0	NULL	LINE integration 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	From this discovery , we propose that LINE ORF1ps play a general role in LINE integration by forming a complex with LINE RNA and rearranging its conformation .
	manualset3
234123	5	428168	15	NULL	NULL	0	NULL	complex	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	From this discovery , we propose that LINE ORF1ps play a general role in LINE integration by forming a complex with LINE RNA and rearranging its conformation .
	manualset3
234124	6	428168	15	NULL	NULL	0	NULL	LINE RNA	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	From this discovery , we propose that LINE ORF1ps play a general role in LINE integration by forming a complex with LINE RNA and rearranging its conformation .
	manualset3
234127	7	428168	15	NULL	NULL	0	NULL	conformation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	From this discovery , we propose that LINE ORF1ps play a general role in LINE integration by forming a complex with LINE RNA and rearranging its conformation .
	manualset3
234128	1	428169	15	NULL	NULL	0	NULL	layer 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	From this layer four strains of spirilloid purple bacteria were isolated , all of which were extremely halophilic .
	manualset3
234129	2	428169	15	NULL	NULL	0	NULL	four strains	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	From this layer four strains of spirilloid purple bacteria were isolated , all of which were extremely halophilic .
	manualset3
234130	3	428169	15	NULL	NULL	0	NULL	spirilloid purple bacteria 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	From this layer four strains of spirilloid purple bacteria were isolated , all of which were extremely halophilic .
	manualset3
234133	1	428170	15	NULL	NULL	0	NULL	series	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	From this series of N-acyltryptamines the 2-bromo derivative ( 5 c ) retains the interesting efficacy profile of 5-HEAT and shows increased melatonin receptor affinities ; it represents one of the first examples of a high-affinity MT ( 1 ) agonist/MT ( 2 ) antagonist .
	manualset3
234134	2	428170	15	NULL	NULL	0	NULL	N-acyltryptamines	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	From this series of N-acyltryptamines the 2-bromo derivative ( 5 c ) retains the interesting efficacy profile of 5-HEAT and shows increased melatonin receptor affinities ; it represents one of the first examples of a high-affinity MT ( 1 ) agonist/MT ( 2 ) antagonist .
	manualset3
234135	3	428170	15	NULL	NULL	0	NULL	2-bromo derivative ( 5 c ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	From this series of N-acyltryptamines the 2-bromo derivative ( 5 c ) retains the interesting efficacy profile of 5-HEAT and shows increased melatonin receptor affinities ; it represents one of the first examples of a high-affinity MT ( 1 ) agonist/MT ( 2 ) antagonist .
	manualset3
234136	4	428170	15	NULL	NULL	0	NULL	efficacy profile	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	From this series of N-acyltryptamines the 2-bromo derivative ( 5 c ) retains the interesting efficacy profile of 5-HEAT and shows increased melatonin receptor affinities ; it represents one of the first examples of a high-affinity MT ( 1 ) agonist/MT ( 2 ) antagonist .
	manualset3
234138	5	428170	15	NULL	NULL	0	NULL	5-HEAT	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	From this series of N-acyltryptamines the 2-bromo derivative ( 5 c ) retains the interesting efficacy profile of 5-HEAT and shows increased melatonin receptor affinities ; it represents one of the first examples of a high-affinity MT ( 1 ) agonist/MT ( 2 ) antagonist .
	manualset3
234141	6	428170	15	NULL	NULL	NULL	NULL	melatonin receptor affinities	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From this series of N-acyltryptamines the 2-bromo derivative ( 5 c ) retains the interesting efficacy profile of 5-HEAT and shows increased melatonin receptor affinities ; it represents one of the first examples of a high-affinity MT ( 1 ) agonist/MT ( 2 ) antagonist .
	manualset3
234142	7	428170	15	NULL	NULL	0	NULL	one	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	From this series of N-acyltryptamines the 2-bromo derivative ( 5 c ) retains the interesting efficacy profile of 5-HEAT and shows increased melatonin receptor affinities ; it represents one of the first examples of a high-affinity MT ( 1 ) agonist/MT ( 2 ) antagonist .
	manualset3
234143	8	428170	15	NULL	NULL	0	NULL	first examples	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	From this series of N-acyltryptamines the 2-bromo derivative ( 5 c ) retains the interesting efficacy profile of 5-HEAT and shows increased melatonin receptor affinities ; it represents one of the first examples of a high-affinity MT ( 1 ) agonist/MT ( 2 ) antagonist .
	manualset3
234151	9	428170	15	NULL	NULL	NULL	NULL	MT ( 1 ) agonist	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From this series of N-acyltryptamines the 2-bromo derivative ( 5 c ) retains the interesting efficacy profile of 5-HEAT and shows increased melatonin receptor affinities ; it represents one of the first examples of a high-affinity MT ( 1 ) agonist/MT ( 2 ) antagonist .
	manualset3
234153	10	428170	15	NULL	NULL	NULL	NULL	MT ( 2 ) antagonist 	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From this series of N-acyltryptamines the 2-bromo derivative ( 5 c ) retains the interesting efficacy profile of 5-HEAT and shows increased melatonin receptor affinities ; it represents one of the first examples of a high-affinity MT ( 1 ) agonist/MT ( 2 ) antagonist .
	manualset3
234173	1	428171	15	NULL	NULL	0	NULL	wk 2 to 17	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	From wk 2 to 17 , the abundance of erm ( T ) and erm ( X ) increased ( P & lt ; 0.05 ) , whereas that of erm ( B ) and erm ( F ) did not .
	manualset3
234176	3	428171	15	NULL	NULL	NULL	NULL	erm ( T )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From wk 2 to 17 , the abundance of erm ( T ) and erm ( X ) increased ( P & lt ; 0.05 ) , whereas that of erm ( B ) and erm ( F ) did not .
	manualset3
234177	4	428171	15	NULL	NULL	NULL	NULL	erm ( X )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From wk 2 to 17 , the abundance of erm ( T ) and erm ( X ) increased ( P & lt ; 0.05 ) , whereas that of erm ( B ) and erm ( F ) did not .
	manualset3
234179	5	428171	15	NULL	NULL	NULL	NULL	P & lt ; 0.05	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From wk 2 to 17 , the abundance of erm ( T ) and erm ( X ) increased ( P & lt ; 0.05 ) , whereas that of erm ( B ) and erm ( F ) did not .
	manualset3
234181	6	428171	15	NULL	NULL	NULL	NULL	erm ( B )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From wk 2 to 17 , the abundance of erm ( T ) and erm ( X ) increased ( P & lt ; 0.05 ) , whereas that of erm ( B ) and erm ( F ) did not .
	manualset3
234183	7	428171	15	NULL	NULL	NULL	NULL	erm ( F ) 	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	From wk 2 to 17 , the abundance of erm ( T ) and erm ( X ) increased ( P & lt ; 0.05 ) , whereas that of erm ( B ) and erm ( F ) did not .
	manualset3
234188	2	428171	15	NULL	NULL	0	NULL	abundance	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	From wk 2 to 17 , the abundance of erm ( T ) and erm ( X ) increased ( P & lt ; 0.05 ) , whereas that of erm ( B ) and erm ( F ) did not .
	manualset3
234191	1	428172	15	NULL	NULL	0	NULL	Frondoside A	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Frondoside A ( 0.01-5 M ) decreased the viability of breast cancer cells in a concentration - and time-dependent manner , with 50 % - effective concentration ( EC50 ) of 2.5 M at 24h .
	manualset3
234192	2	428172	15	NULL	NULL	0	NULL	0.01-5 M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Frondoside A ( 0.01-5 M ) decreased the viability of breast cancer cells in a concentration - and time-dependent manner , with 50 % - effective concentration ( EC50 ) of 2.5 M at 24h .
	manualset3
234193	3	428172	15	NULL	NULL	0	NULL	viability	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Frondoside A ( 0.01-5 M ) decreased the viability of breast cancer cells in a concentration - and time-dependent manner , with 50 % - effective concentration ( EC50 ) of 2.5 M at 24h .
	manualset3
234194	4	428172	15	NULL	NULL	0	NULL	breast cancer cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Frondoside A ( 0.01-5 M ) decreased the viability of breast cancer cells in a concentration - and time-dependent manner , with 50 % - effective concentration ( EC50 ) of 2.5 M at 24h .
	manualset3
234195	5	428172	15	NULL	NULL	NULL	NULL	concentration dependent manner	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Frondoside A ( 0.01-5 M ) decreased the viability of breast cancer cells in a concentration - and time-dependent manner , with 50 % - effective concentration ( EC50 ) of 2.5 M at 24h .
	manualset3
234196	6	428172	15	NULL	NULL	0	NULL	time-dependent manner	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Frondoside A ( 0.01-5 M ) decreased the viability of breast cancer cells in a concentration - and time-dependent manner , with 50 % - effective concentration ( EC50 ) of 2.5 M at 24h .
	manualset3
234197	7	428172	15	NULL	NULL	0	NULL	50 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Frondoside A ( 0.01-5 M ) decreased the viability of breast cancer cells in a concentration - and time-dependent manner , with 50 % - effective concentration ( EC50 ) of 2.5 M at 24h .
	manualset3
234198	8	428172	15	NULL	NULL	0	NULL	effective concentration ( EC50 )	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Frondoside A ( 0.01-5 M ) decreased the viability of breast cancer cells in a concentration - and time-dependent manner , with 50 % - effective concentration ( EC50 ) of 2.5 M at 24h .
	manualset3
234199	9	428172	15	NULL	NULL	0	NULL	2.5 M	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Frondoside A ( 0.01-5 M ) decreased the viability of breast cancer cells in a concentration - and time-dependent manner , with 50 % - effective concentration ( EC50 ) of 2.5 M at 24h .
	manualset3
234200	10	428172	15	NULL	NULL	0	NULL	24h	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Frondoside A ( 0.01-5 M ) decreased the viability of breast cancer cells in a concentration - and time-dependent manner , with 50 % - effective concentration ( EC50 ) of 2.5 M at 24h .
	manualset3
234201	1	428173	15	NULL	NULL	0	NULL	Frontotemporal Lobar degeneration ( FTLD )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Frontotemporal Lobar degeneration ( FTLD ) is one of the most important neurodegenerative conditions , affecting in the presenium , but more recently recognized also in aged population .
	manualset3
234202	2	428173	15	NULL	NULL	0	NULL	one 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Frontotemporal Lobar degeneration ( FTLD ) is one of the most important neurodegenerative conditions , affecting in the presenium , but more recently recognized also in aged population .
	manualset3
234203	3	428173	15	NULL	NULL	0	NULL	neurodegenerative conditions	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Frontotemporal Lobar degeneration ( FTLD ) is one of the most important neurodegenerative conditions , affecting in the presenium , but more recently recognized also in aged population .
	manualset3
234204	4	428173	15	NULL	NULL	0	NULL	presenium	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Frontotemporal Lobar degeneration ( FTLD ) is one of the most important neurodegenerative conditions , affecting in the presenium , but more recently recognized also in aged population .
	manualset3
234205	5	428173	15	NULL	NULL	0	NULL	aged population 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Frontotemporal Lobar degeneration ( FTLD ) is one of the most important neurodegenerative conditions , affecting in the presenium , but more recently recognized also in aged population .
	manualset3
234206	1	428174	15	NULL	NULL	0	NULL	Admission diagnosis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Admission diagnosis in tubal pregnancy ) .
	manualset3
234207	2	428174	15	NULL	NULL	0	NULL	tubal pregnancy	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Admission diagnosis in tubal pregnancy ) .
	manualset3
234208	1	428175	15	NULL	NULL	0	NULL	Risk of infection	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Risk of infection by biologics ) .
	manualset3
234210	2	428175	15	NULL	NULL	0	NULL	biologics	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	( Risk of infection by biologics ) .
	manualset3
234211	1	428176	15	NULL	NULL	0	NULL	Frontotemporal lobar degeneration ( FTLD )	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Frontotemporal lobar degeneration ( FTLD ) - TDP type 3 pathology was found at autopsy .
	manualset3
234212	2	428176	15	NULL	NULL	0	NULL	TDP type 3 pathology	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Frontotemporal lobar degeneration ( FTLD ) - TDP type 3 pathology was found at autopsy .
	manualset3
234213	3	428176	15	NULL	NULL	0	NULL	autopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Frontotemporal lobar degeneration ( FTLD ) - TDP type 3 pathology was found at autopsy .
	manualset3
234214	1	428177	15	NULL	NULL	NULL	NULL	Frozen biopsy material 	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Frozen biopsy material was obtained from 13 patients with LCH and 20 patients without the disease .
	manualset3
234215	2	428177	15	NULL	NULL	0	NULL	13 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Frozen biopsy material was obtained from 13 patients with LCH and 20 patients without the disease .
	manualset3
234217	3	428177	15	NULL	NULL	0	NULL	LCH	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Frozen biopsy material was obtained from 13 patients with LCH and 20 patients without the disease .
	manualset3
234218	4	428177	15	NULL	NULL	0	NULL	20 patients	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Frozen biopsy material was obtained from 13 patients with LCH and 20 patients without the disease .
	manualset3
234219	5	428177	15	NULL	NULL	0	NULL	disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Frozen biopsy material was obtained from 13 patients with LCH and 20 patients without the disease .
	manualset3
234225	1	428178	15	NULL	NULL	0	NULL	Fructose 1 , 6-diphosphate ( FDP ) aldolase 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Fructose 1 , 6-diphosphate ( FDP ) aldolase and 2-keto-3-deoxy-D-gluconate ( KDG ) aldolase the two key enzymes of Embden-Meyerhof-Parnas ( EMP ) and the nonphosphorolytic Entner-Doudoroff ( ED ) pathways respectively , were identified in cell-free extracts of four Aspergillus oryzae strains grown on D-glucose as sole source of carbon .
	manualset3
234226	2	428178	15	NULL	NULL	0	NULL	2-keto-3-deoxy-D-gluconate ( KDG ) aldolase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Fructose 1 , 6-diphosphate ( FDP ) aldolase and 2-keto-3-deoxy-D-gluconate ( KDG ) aldolase the two key enzymes of Embden-Meyerhof-Parnas ( EMP ) and the nonphosphorolytic Entner-Doudoroff ( ED ) pathways respectively , were identified in cell-free extracts of four Aspergillus oryzae strains grown on D-glucose as sole source of carbon .
	manualset3
234227	3	428178	15	NULL	NULL	0	NULL	two 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Fructose 1 , 6-diphosphate ( FDP ) aldolase and 2-keto-3-deoxy-D-gluconate ( KDG ) aldolase the two key enzymes of Embden-Meyerhof-Parnas ( EMP ) and the nonphosphorolytic Entner-Doudoroff ( ED ) pathways respectively , were identified in cell-free extracts of four Aspergillus oryzae strains grown on D-glucose as sole source of carbon .
	manualset3
234229	4	428178	15	NULL	NULL	NULL	NULL	enzymes 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fructose 1 , 6-diphosphate ( FDP ) aldolase and 2-keto-3-deoxy-D-gluconate ( KDG ) aldolase the two key enzymes of Embden-Meyerhof-Parnas ( EMP ) and the nonphosphorolytic Entner-Doudoroff ( ED ) pathways respectively , were identified in cell-free extracts of four Aspergillus oryzae strains grown on D-glucose as sole source of carbon .
	manualset3
234231	5	428178	15	NULL	NULL	0	NULL	Embden-Meyerhof-Parnas ( EMP ) pathway	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fructose 1 , 6-diphosphate ( FDP ) aldolase and 2-keto-3-deoxy-D-gluconate ( KDG ) aldolase the two key enzymes of Embden-Meyerhof-Parnas ( EMP ) and the nonphosphorolytic Entner-Doudoroff ( ED ) pathways respectively , were identified in cell-free extracts of four Aspergillus oryzae strains grown on D-glucose as sole source of carbon .
	manualset3
234232	6	428178	15	NULL	NULL	0	NULL	nonphosphorolytic Entner-Doudoroff ( ED ) pathways	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fructose 1 , 6-diphosphate ( FDP ) aldolase and 2-keto-3-deoxy-D-gluconate ( KDG ) aldolase the two key enzymes of Embden-Meyerhof-Parnas ( EMP ) and the nonphosphorolytic Entner-Doudoroff ( ED ) pathways respectively , were identified in cell-free extracts of four Aspergillus oryzae strains grown on D-glucose as sole source of carbon .
	manualset3
234234	7	428178	15	NULL	NULL	0	NULL	cell-free extracts	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Fructose 1 , 6-diphosphate ( FDP ) aldolase and 2-keto-3-deoxy-D-gluconate ( KDG ) aldolase the two key enzymes of Embden-Meyerhof-Parnas ( EMP ) and the nonphosphorolytic Entner-Doudoroff ( ED ) pathways respectively , were identified in cell-free extracts of four Aspergillus oryzae strains grown on D-glucose as sole source of carbon .
	manualset3
234235	8	428178	15	NULL	NULL	0	NULL	four 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Fructose 1 , 6-diphosphate ( FDP ) aldolase and 2-keto-3-deoxy-D-gluconate ( KDG ) aldolase the two key enzymes of Embden-Meyerhof-Parnas ( EMP ) and the nonphosphorolytic Entner-Doudoroff ( ED ) pathways respectively , were identified in cell-free extracts of four Aspergillus oryzae strains grown on D-glucose as sole source of carbon .
	manualset3
234236	9	428178	15	NULL	NULL	0	NULL	Aspergillus oryzae strains	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Fructose 1 , 6-diphosphate ( FDP ) aldolase and 2-keto-3-deoxy-D-gluconate ( KDG ) aldolase the two key enzymes of Embden-Meyerhof-Parnas ( EMP ) and the nonphosphorolytic Entner-Doudoroff ( ED ) pathways respectively , were identified in cell-free extracts of four Aspergillus oryzae strains grown on D-glucose as sole source of carbon .
	manualset3
234237	10	428178	15	NULL	NULL	0	NULL	D-glucose	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Fructose 1 , 6-diphosphate ( FDP ) aldolase and 2-keto-3-deoxy-D-gluconate ( KDG ) aldolase the two key enzymes of Embden-Meyerhof-Parnas ( EMP ) and the nonphosphorolytic Entner-Doudoroff ( ED ) pathways respectively , were identified in cell-free extracts of four Aspergillus oryzae strains grown on D-glucose as sole source of carbon .
	manualset3
234238	11	428178	15	NULL	NULL	NULL	NULL	source 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fructose 1 , 6-diphosphate ( FDP ) aldolase and 2-keto-3-deoxy-D-gluconate ( KDG ) aldolase the two key enzymes of Embden-Meyerhof-Parnas ( EMP ) and the nonphosphorolytic Entner-Doudoroff ( ED ) pathways respectively , were identified in cell-free extracts of four Aspergillus oryzae strains grown on D-glucose as sole source of carbon .
	manualset3
234239	12	428178	15	NULL	NULL	0	NULL	carbon	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Fructose 1 , 6-diphosphate ( FDP ) aldolase and 2-keto-3-deoxy-D-gluconate ( KDG ) aldolase the two key enzymes of Embden-Meyerhof-Parnas ( EMP ) and the nonphosphorolytic Entner-Doudoroff ( ED ) pathways respectively , were identified in cell-free extracts of four Aspergillus oryzae strains grown on D-glucose as sole source of carbon .
	manualset3
234242	2	428179	15	NULL	NULL	NULL	NULL	protein	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Frugal cooking : getting your protein .
	manualset3
234245	1	428179	15	NULL	NULL	0	NULL	cooking	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Frugal cooking : getting your protein .
	manualset3
234247	1	428180	15	NULL	NULL	0	NULL	Fruit intake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Fruit and vegetable intake and survival from non-Hodgkin lymphoma : does an apple a day keep the doctor away ?
	manualset3
234248	2	428180	15	NULL	NULL	0	NULL	vegetable intake	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Fruit and vegetable intake and survival from non-Hodgkin lymphoma : does an apple a day keep the doctor away ?
	manualset3
234250	3	428180	15	NULL	NULL	0	NULL	survival 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fruit and vegetable intake and survival from non-Hodgkin lymphoma : does an apple a day keep the doctor away ?
	manualset3
234251	4	428180	15	NULL	NULL	0	NULL	non-Hodgkin lymphoma	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Fruit and vegetable intake and survival from non-Hodgkin lymphoma : does an apple a day keep the doctor away ?
	manualset3
234252	5	428180	15	NULL	NULL	0	NULL	apple 	Food												NULL		0	NULL	NULL	NULL	NULL	NULL	Fruit and vegetable intake and survival from non-Hodgkin lymphoma : does an apple a day keep the doctor away ?
	manualset3
234253	6	428180	15	NULL	NULL	0	NULL	doctor	Person												NULL		0	NULL	NULL	NULL	NULL	NULL	Fruit and vegetable intake and survival from non-Hodgkin lymphoma : does an apple a day keep the doctor away ?
	manualset3
234255	1	428181	15	NULL	NULL	0	NULL	FtsZ 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	FtsZ is an attractive target for the development of new antibiotics .
	manualset3
234256	2	428181	15	NULL	NULL	NULL	NULL	target	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	FtsZ is an attractive target for the development of new antibiotics .
	manualset3
234257	3	428181	15	NULL	NULL	NULL	NULL	development 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	FtsZ is an attractive target for the development of new antibiotics .
	manualset3
234258	4	428181	15	NULL	NULL	0	NULL	antibiotics 	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	FtsZ is an attractive target for the development of new antibiotics .
	manualset3
234260	1	428182	15	NULL	NULL	0	NULL	Fukuyama-type congenital muscular dystrophy ( FCMD )	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Fukuyama-type congenital muscular dystrophy ( FCMD ) , the second most common childhood muscular dystrophy in Japan , is caused by alterations in the fukutin gene .
	manualset3
234262	2	428182	15	NULL	NULL	NULL	NULL	childhood muscular dystrophy	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fukuyama-type congenital muscular dystrophy ( FCMD ) , the second most common childhood muscular dystrophy in Japan , is caused by alterations in the fukutin gene .
	manualset3
234264	3	428182	15	NULL	NULL	NULL	NULL	Japan	ProperNamedGeographicalLocation												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fukuyama-type congenital muscular dystrophy ( FCMD ) , the second most common childhood muscular dystrophy in Japan , is caused by alterations in the fukutin gene .
	manualset3
234265	4	428182	15	NULL	NULL	NULL	NULL	alterations 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fukuyama-type congenital muscular dystrophy ( FCMD ) , the second most common childhood muscular dystrophy in Japan , is caused by alterations in the fukutin gene .
	manualset3
234266	5	428182	15	NULL	NULL	NULL	NULL	fukutin gene	Gene												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fukuyama-type congenital muscular dystrophy ( FCMD ) , the second most common childhood muscular dystrophy in Japan , is caused by alterations in the fukutin gene .
	manualset3
234272	1	428183	15	NULL	NULL	0	NULL	thickness	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Full-thickness , excisional wound healing in healthy BALB/c mice was significantly accelerated by daily topical application of NABPs such as guanosine ( 50 % closure by days 2.5-2 .8 ) .
	manualset3
234274	2	428183	15	NULL	NULL	0	NULL	excisional wound healing	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Full-thickness , excisional wound healing in healthy BALB/c mice was significantly accelerated by daily topical application of NABPs such as guanosine ( 50 % closure by days 2.5-2 .8 ) .
	manualset3
234276	3	428183	15	NULL	NULL	0	NULL	BALB/c mice 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Full-thickness , excisional wound healing in healthy BALB/c mice was significantly accelerated by daily topical application of NABPs such as guanosine ( 50 % closure by days 2.5-2 .8 ) .
	manualset3
234278	4	428183	15	NULL	NULL	0	NULL	daily	Time												NULL		0	NULL	NULL	NULL	NULL	NULL	Full-thickness , excisional wound healing in healthy BALB/c mice was significantly accelerated by daily topical application of NABPs such as guanosine ( 50 % closure by days 2.5-2 .8 ) .
	manualset3
234279	5	428183	15	NULL	NULL	NULL	NULL	topical application	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Full-thickness , excisional wound healing in healthy BALB/c mice was significantly accelerated by daily topical application of NABPs such as guanosine ( 50 % closure by days 2.5-2 .8 ) .
	manualset3
234282	6	428183	15	NULL	NULL	0	NULL	NABPs	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Full-thickness , excisional wound healing in healthy BALB/c mice was significantly accelerated by daily topical application of NABPs such as guanosine ( 50 % closure by days 2.5-2 .8 ) .
	manualset3
234283	7	428183	15	NULL	NULL	0	NULL	guanosine 	NucleicAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Full-thickness , excisional wound healing in healthy BALB/c mice was significantly accelerated by daily topical application of NABPs such as guanosine ( 50 % closure by days 2.5-2 .8 ) .
	manualset3
234290	8	428183	15	NULL	NULL	0	NULL	50 % closure	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Full-thickness , excisional wound healing in healthy BALB/c mice was significantly accelerated by daily topical application of NABPs such as guanosine ( 50 % closure by days 2.5-2 .8 ) .
	manualset3
234296	9	428183	15	NULL	NULL	NULL	NULL	days 2.5-2 .8	Duration												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Full-thickness , excisional wound healing in healthy BALB/c mice was significantly accelerated by daily topical application of NABPs such as guanosine ( 50 % closure by days 2.5-2 .8 ) .
	manualset3
234315	1	428184	15	NULL	NULL	0	NULL	Risk of thrombosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Risk of thrombosis in prolonged catheterization of the radial artery : comparison of 2 types of catheters ) .
	manualset3
234317	2	428184	15	NULL	NULL	0	NULL	catheterization of the radial artery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Risk of thrombosis in prolonged catheterization of the radial artery : comparison of 2 types of catheters ) .
	manualset3
234320	3	428184	15	NULL	NULL	0	NULL	comparison	Relationship												NULL		0	NULL	NULL	NULL	NULL	NULL	( Risk of thrombosis in prolonged catheterization of the radial artery : comparison of 2 types of catheters ) .
	manualset3
234321	4	428184	15	NULL	NULL	0	NULL	2 types	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	( Risk of thrombosis in prolonged catheterization of the radial artery : comparison of 2 types of catheters ) .
	manualset3
234322	5	428184	15	NULL	NULL	0	NULL	catheters	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	( Risk of thrombosis in prolonged catheterization of the radial artery : comparison of 2 types of catheters ) .
	manualset3
234349	1	428185	15	NULL	NULL	0	NULL	Fullerene C ( 60 ) 	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Fullerene C ( 60 ) was also detected by ELISA in organ homogenates of rats intraperitoneally or intragastrically administered with fullerene .
	manualset3
234350	2	428185	15	NULL	NULL	0	NULL	ELISA	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Fullerene C ( 60 ) was also detected by ELISA in organ homogenates of rats intraperitoneally or intragastrically administered with fullerene .
	manualset3
234352	3	428185	15	NULL	NULL	0	NULL	organ homogenates	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Fullerene C ( 60 ) was also detected by ELISA in organ homogenates of rats intraperitoneally or intragastrically administered with fullerene .
	manualset3
234354	4	428185	15	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Fullerene C ( 60 ) was also detected by ELISA in organ homogenates of rats intraperitoneally or intragastrically administered with fullerene .
	manualset3
234363	5	428185	15	NULL	NULL	NULL	NULL	fullerene	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fullerene C ( 60 ) was also detected by ELISA in organ homogenates of rats intraperitoneally or intragastrically administered with fullerene .
	manualset3
234366	1	428186	15	NULL	NULL	0	NULL	Fully matured DCs	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Fully matured DCs are relatively well-defined and even used in clinical trials in cancer .
	manualset3
234367	2	428186	15	NULL	NULL	0	NULL	clinical trials 	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	Fully matured DCs are relatively well-defined and even used in clinical trials in cancer .
	manualset3
234368	3	428186	15	NULL	NULL	0	NULL	cancer 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Fully matured DCs are relatively well-defined and even used in clinical trials in cancer .
	manualset3
234369	1	428187	15	NULL	NULL	NULL	NULL	Functional analyses 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional analyses of multiple atpap10 mutant alleles and overexpressing lines indicated that AtPAP10 plays an important role in plant tolerance to Pi limitation .
	manualset3
234370	2	428187	15	NULL	NULL	NULL	NULL	atpap10 mutant alleles 	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional analyses of multiple atpap10 mutant alleles and overexpressing lines indicated that AtPAP10 plays an important role in plant tolerance to Pi limitation .
	manualset3
234371	3	428187	15	NULL	NULL	0	NULL	overexpressing lines	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional analyses of multiple atpap10 mutant alleles and overexpressing lines indicated that AtPAP10 plays an important role in plant tolerance to Pi limitation .
	manualset3
234372	4	428187	15	NULL	NULL	NULL	NULL	AtPAP10	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional analyses of multiple atpap10 mutant alleles and overexpressing lines indicated that AtPAP10 plays an important role in plant tolerance to Pi limitation .
	manualset3
234373	5	428187	15	NULL	NULL	0	NULL	role	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional analyses of multiple atpap10 mutant alleles and overexpressing lines indicated that AtPAP10 plays an important role in plant tolerance to Pi limitation .
	manualset3
234374	6	428187	15	NULL	NULL	0	NULL	plant tolerance 	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional analyses of multiple atpap10 mutant alleles and overexpressing lines indicated that AtPAP10 plays an important role in plant tolerance to Pi limitation .
	manualset3
234375	7	428187	15	NULL	NULL	0	NULL	Pi limitation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional analyses of multiple atpap10 mutant alleles and overexpressing lines indicated that AtPAP10 plays an important role in plant tolerance to Pi limitation .
	manualset3
234376	2	428188	15	NULL	NULL	NULL	NULL	antiischaemic effects	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional and antiischaemic effects of monoacetyl-vitexinrhamnoside ( AVR ) , a flavonoid with phosphodiesterase ( PDE ) - inhibitory properties contained in Crataegus species ( Hawthorn , Rosaceae ) were studied in several in-vitro models .
	manualset3
234377	3	428188	15	NULL	NULL	NULL	NULL	monoacetyl-vitexinrhamnoside ( AVR ) 	Drug												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional and antiischaemic effects of monoacetyl-vitexinrhamnoside ( AVR ) , a flavonoid with phosphodiesterase ( PDE ) - inhibitory properties contained in Crataegus species ( Hawthorn , Rosaceae ) were studied in several in-vitro models .
	manualset3
234378	4	428188	15	NULL	NULL	NULL	NULL	flavonoid	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional and antiischaemic effects of monoacetyl-vitexinrhamnoside ( AVR ) , a flavonoid with phosphodiesterase ( PDE ) - inhibitory properties contained in Crataegus species ( Hawthorn , Rosaceae ) were studied in several in-vitro models .
	manualset3
234379	5	428188	15	NULL	NULL	NULL	NULL	phosphodiesterase ( PDE ) - inhibitory properties	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional and antiischaemic effects of monoacetyl-vitexinrhamnoside ( AVR ) , a flavonoid with phosphodiesterase ( PDE ) - inhibitory properties contained in Crataegus species ( Hawthorn , Rosaceae ) were studied in several in-vitro models .
	manualset3
234380	6	428188	15	NULL	NULL	NULL	NULL	Crataegus species	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional and antiischaemic effects of monoacetyl-vitexinrhamnoside ( AVR ) , a flavonoid with phosphodiesterase ( PDE ) - inhibitory properties contained in Crataegus species ( Hawthorn , Rosaceae ) were studied in several in-vitro models .
	manualset3
234381	7	428188	15	NULL	NULL	NULL	NULL	Hawthorn , Rosaceae	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional and antiischaemic effects of monoacetyl-vitexinrhamnoside ( AVR ) , a flavonoid with phosphodiesterase ( PDE ) - inhibitory properties contained in Crataegus species ( Hawthorn , Rosaceae ) were studied in several in-vitro models .
	manualset3
234382	8	428188	15	NULL	NULL	NULL	NULL	in-vitro models	IntellectualProduct												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional and antiischaemic effects of monoacetyl-vitexinrhamnoside ( AVR ) , a flavonoid with phosphodiesterase ( PDE ) - inhibitory properties contained in Crataegus species ( Hawthorn , Rosaceae ) were studied in several in-vitro models .
	manualset3
235752	1	428188	15	NULL	NULL	NULL	NULL	Functional effects	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional and antiischaemic effects of monoacetyl-vitexinrhamnoside ( AVR ) , a flavonoid with phosphodiesterase ( PDE ) - inhibitory properties contained in Crataegus species ( Hawthorn , Rosaceae ) were studied in several in-vitro models .
	manualset3
234383	2	428189	15	NULL	NULL	NULL	NULL	biochemical parameters	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional and biochemical parameters such as brain and serum cholinesterase ( ChE ) and liver xenobiotic metabolizing system , including the biotransformation of CPF itself , have been studied and the no observed effect levels ( NOELs ) identified .
	manualset3
234384	3	428189	15	NULL	NULL	NULL	NULL	Brain cholinesterase ( ChE )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional and biochemical parameters such as brain and serum cholinesterase ( ChE ) and liver xenobiotic metabolizing system , including the biotransformation of CPF itself , have been studied and the no observed effect levels ( NOELs ) identified .
	manualset3
234385	4	428189	15	NULL	NULL	NULL	NULL	serum cholinesterase ( ChE )	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional and biochemical parameters such as brain and serum cholinesterase ( ChE ) and liver xenobiotic metabolizing system , including the biotransformation of CPF itself , have been studied and the no observed effect levels ( NOELs ) identified .
	manualset3
234386	5	428189	15	NULL	NULL	NULL	NULL	liver xenobiotic metabolizing system	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional and biochemical parameters such as brain and serum cholinesterase ( ChE ) and liver xenobiotic metabolizing system , including the biotransformation of CPF itself , have been studied and the no observed effect levels ( NOELs ) identified .
	manualset3
234387	6	428189	15	NULL	NULL	NULL	NULL	biotransformation	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional and biochemical parameters such as brain and serum cholinesterase ( ChE ) and liver xenobiotic metabolizing system , including the biotransformation of CPF itself , have been studied and the no observed effect levels ( NOELs ) identified .
	manualset3
234388	7	428189	15	NULL	NULL	NULL	NULL	CPF	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional and biochemical parameters such as brain and serum cholinesterase ( ChE ) and liver xenobiotic metabolizing system , including the biotransformation of CPF itself , have been studied and the no observed effect levels ( NOELs ) identified .
	manualset3
234389	8	428189	15	NULL	NULL	NULL	NULL	no observed effect levels ( NOELs )	Quantity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional and biochemical parameters such as brain and serum cholinesterase ( ChE ) and liver xenobiotic metabolizing system , including the biotransformation of CPF itself , have been studied and the no observed effect levels ( NOELs ) identified .
	manualset3
235753	1	428189	15	NULL	NULL	0	NULL	Functional parameters 	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional and biochemical parameters such as brain and serum cholinesterase ( ChE ) and liver xenobiotic metabolizing system , including the biotransformation of CPF itself , have been studied and the no observed effect levels ( NOELs ) identified .
	manualset3
234390	2	428190	15	NULL	NULL	NULL	NULL	structural characterization	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional and structural characterization of isolated perfused stingray liver including effects of ischaemia/reperfusion .
	manualset3
234391	4	428190	15	NULL	NULL	NULL	NULL	liver	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional and structural characterization of isolated perfused stingray liver including effects of ischaemia/reperfusion .
	manualset3
234392	6	428190	15	NULL	NULL	NULL	NULL	ischaemia	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional and structural characterization of isolated perfused stingray liver including effects of ischaemia/reperfusion .
	manualset3
234393	7	428190	15	NULL	NULL	NULL	NULL	reperfusion	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional and structural characterization of isolated perfused stingray liver including effects of ischaemia/reperfusion .
	manualset3
234394	3	428190	15	NULL	NULL	NULL	NULL	stingray 	Organism												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional and structural characterization of isolated perfused stingray liver including effects of ischaemia/reperfusion .
	manualset3
234395	5	428190	15	NULL	NULL	NULL	NULL	effects 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional and structural characterization of isolated perfused stingray liver including effects of ischaemia/reperfusion .
	manualset3
235755	1	428190	15	NULL	NULL	0	NULL	Functional characterization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional and structural characterization of isolated perfused stingray liver including effects of ischaemia/reperfusion .
	manualset3
234405	1	428191	15	NULL	NULL	0	NULL	characterization	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional characterization of a trafficking-defective HCN4 mutation , D553N , associated with cardiac arrhythmia .
	manualset3
234406	2	428191	15	NULL	NULL	0	NULL	HCN4 mutation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional characterization of a trafficking-defective HCN4 mutation , D553N , associated with cardiac arrhythmia .
	manualset3
234407	3	428191	15	NULL	NULL	NULL	NULL	D553N	AminoAcid												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional characterization of a trafficking-defective HCN4 mutation , D553N , associated with cardiac arrhythmia .
	manualset3
234408	4	428191	15	NULL	NULL	0	NULL	cardiac arrhythmia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional characterization of a trafficking-defective HCN4 mutation , D553N , associated with cardiac arrhythmia .
	manualset3
234409	1	428192	15	NULL	NULL	0	NULL	dyspepsia 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional dyspepsia -- defined as chronic or recurrent pain or discomfort centred in the upper abdomen , with no clinical or endoscopic evidence of known organic disease -- is very common and causes considerable morbidity and loss of productivity .
	manualset3
234410	2	428192	15	NULL	NULL	NULL	NULL	chronic pain 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional dyspepsia -- defined as chronic or recurrent pain or discomfort centred in the upper abdomen , with no clinical or endoscopic evidence of known organic disease -- is very common and causes considerable morbidity and loss of productivity .
	manualset3
234411	4	428192	15	NULL	NULL	NULL	NULL	discomfort	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional dyspepsia -- defined as chronic or recurrent pain or discomfort centred in the upper abdomen , with no clinical or endoscopic evidence of known organic disease -- is very common and causes considerable morbidity and loss of productivity .
	manualset3
234412	5	428192	15	NULL	NULL	NULL	NULL	upper abdomen	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional dyspepsia -- defined as chronic or recurrent pain or discomfort centred in the upper abdomen , with no clinical or endoscopic evidence of known organic disease -- is very common and causes considerable morbidity and loss of productivity .
	manualset3
234413	6	428192	15	NULL	NULL	NULL	NULL	clinical evidence 	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional dyspepsia -- defined as chronic or recurrent pain or discomfort centred in the upper abdomen , with no clinical or endoscopic evidence of known organic disease -- is very common and causes considerable morbidity and loss of productivity .
	manualset3
234414	8	428192	15	NULL	NULL	NULL	NULL	organic disease	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional dyspepsia -- defined as chronic or recurrent pain or discomfort centred in the upper abdomen , with no clinical or endoscopic evidence of known organic disease -- is very common and causes considerable morbidity and loss of productivity .
	manualset3
234415	9	428192	15	NULL	NULL	NULL	NULL	morbidity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional dyspepsia -- defined as chronic or recurrent pain or discomfort centred in the upper abdomen , with no clinical or endoscopic evidence of known organic disease -- is very common and causes considerable morbidity and loss of productivity .
	manualset3
234416	10	428192	15	NULL	NULL	NULL	NULL	loss of productivity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional dyspepsia -- defined as chronic or recurrent pain or discomfort centred in the upper abdomen , with no clinical or endoscopic evidence of known organic disease -- is very common and causes considerable morbidity and loss of productivity .
	manualset3
235756	3	428192	15	NULL	NULL	0	NULL	recurrent pain	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional dyspepsia -- defined as chronic or recurrent pain or discomfort centred in the upper abdomen , with no clinical or endoscopic evidence of known organic disease -- is very common and causes considerable morbidity and loss of productivity .
	manualset3
235757	7	428192	15	NULL	NULL	0	NULL	endoscopic evidence	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional dyspepsia -- defined as chronic or recurrent pain or discomfort centred in the upper abdomen , with no clinical or endoscopic evidence of known organic disease -- is very common and causes considerable morbidity and loss of productivity .
	manualset3
234419	1	428193	15	NULL	NULL	NULL	NULL	Functional interaction	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional interaction of NMDA and group I metabotropic glutamate receptors in negatively reinforced learning in rats .
	manualset3
234420	2	428193	15	NULL	NULL	NULL	NULL	NMDA receptors	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional interaction of NMDA and group I metabotropic glutamate receptors in negatively reinforced learning in rats .
	manualset3
234421	3	428193	15	NULL	NULL	NULL	NULL	group I metabotropic glutamate receptors	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional interaction of NMDA and group I metabotropic glutamate receptors in negatively reinforced learning in rats .
	manualset3
234422	4	428193	15	NULL	NULL	0	NULL	learning	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional interaction of NMDA and group I metabotropic glutamate receptors in negatively reinforced learning in rats .
	manualset3
234423	5	428193	15	NULL	NULL	0	NULL	rats	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional interaction of NMDA and group I metabotropic glutamate receptors in negatively reinforced learning in rats .
	manualset3
234424	1	428194	15	NULL	NULL	0	NULL	interpretations	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional interpretations of sadness , stress and demoralization among an urban population of low-income mothers .
	manualset3
234425	2	428194	15	NULL	NULL	0	NULL	sadness	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional interpretations of sadness , stress and demoralization among an urban population of low-income mothers .
	manualset3
234426	3	428194	15	NULL	NULL	0	NULL	stress	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional interpretations of sadness , stress and demoralization among an urban population of low-income mothers .
	manualset3
234427	4	428194	15	NULL	NULL	0	NULL	demoralization 	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional interpretations of sadness , stress and demoralization among an urban population of low-income mothers .
	manualset3
234428	5	428194	15	NULL	NULL	0	NULL	urban population	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional interpretations of sadness , stress and demoralization among an urban population of low-income mothers .
	manualset3
234429	6	428194	15	NULL	NULL	0	NULL	low-income mothers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional interpretations of sadness , stress and demoralization among an urban population of low-income mothers .
	manualset3
234432	1	428195	15	NULL	NULL	0	NULL	properties	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional properties of mahaim fibers .
	manualset3
234433	2	428195	15	NULL	NULL	0	NULL	mahaim fibers	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional properties of mahaim fibers .
	manualset3
234434	1	428196	15	NULL	NULL	NULL	NULL	Functional radiography	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional radiography or MRI was also necessary , as plain radiographs and CT scan failed to detect significant ligamentous injuries in 6 % of the patients .
	manualset3
234435	2	428196	15	NULL	NULL	0	NULL	MRI	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional radiography or MRI was also necessary , as plain radiographs and CT scan failed to detect significant ligamentous injuries in 6 % of the patients .
	manualset3
234438	3	428196	15	NULL	NULL	NULL	NULL	radiographs	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional radiography or MRI was also necessary , as plain radiographs and CT scan failed to detect significant ligamentous injuries in 6 % of the patients .
	manualset3
234439	4	428196	15	NULL	NULL	NULL	NULL	CT scan	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional radiography or MRI was also necessary , as plain radiographs and CT scan failed to detect significant ligamentous injuries in 6 % of the patients .
	manualset3
234442	6	428196	15	NULL	NULL	NULL	NULL	6 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional radiography or MRI was also necessary , as plain radiographs and CT scan failed to detect significant ligamentous injuries in 6 % of the patients .
	manualset3
234443	7	428196	15	NULL	NULL	NULL	NULL	patients	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional radiography or MRI was also necessary , as plain radiographs and CT scan failed to detect significant ligamentous injuries in 6 % of the patients .
	manualset3
235758	5	428196	15	NULL	NULL	NULL	NULL	ligamentous injuries	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional radiography or MRI was also necessary , as plain radiographs and CT scan failed to detect significant ligamentous injuries in 6 % of the patients .
	manualset3
234447	1	428197	15	NULL	NULL	0	NULL	recovery 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional recovery , expressed as a percentage of prearrest LVF , was 38.1 % + / - 10.7 % in group 1 and 84.0 % + / - 8.1 % in group 4 ( p less than 0.008 ) .
	manualset3
234448	2	428197	15	NULL	NULL	0	NULL	percentage	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional recovery , expressed as a percentage of prearrest LVF , was 38.1 % + / - 10.7 % in group 1 and 84.0 % + / - 8.1 % in group 4 ( p less than 0.008 ) .
	manualset3
234449	3	428197	15	NULL	NULL	0	NULL	prearrest LVF	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional recovery , expressed as a percentage of prearrest LVF , was 38.1 % + / - 10.7 % in group 1 and 84.0 % + / - 8.1 % in group 4 ( p less than 0.008 ) .
	manualset3
234451	4	428197	15	NULL	NULL	0	NULL	38.1 % + / - 10.7 %	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional recovery , expressed as a percentage of prearrest LVF , was 38.1 % + / - 10.7 % in group 1 and 84.0 % + / - 8.1 % in group 4 ( p less than 0.008 ) .
	manualset3
234458	5	428197	15	NULL	NULL	0	NULL	group 1	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional recovery , expressed as a percentage of prearrest LVF , was 38.1 % + / - 10.7 % in group 1 and 84.0 % + / - 8.1 % in group 4 ( p less than 0.008 ) .
	manualset3
234460	6	428197	15	NULL	NULL	0	NULL	84.0 % + / - 8.1 % 	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional recovery , expressed as a percentage of prearrest LVF , was 38.1 % + / - 10.7 % in group 1 and 84.0 % + / - 8.1 % in group 4 ( p less than 0.008 ) .
	manualset3
234461	7	428197	15	NULL	NULL	0	NULL	group 4 	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional recovery , expressed as a percentage of prearrest LVF , was 38.1 % + / - 10.7 % in group 1 and 84.0 % + / - 8.1 % in group 4 ( p less than 0.008 ) .
	manualset3
234462	8	428197	15	NULL	NULL	0	NULL	p less than 0.008	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional recovery , expressed as a percentage of prearrest LVF , was 38.1 % + / - 10.7 % in group 1 and 84.0 % + / - 8.1 % in group 4 ( p less than 0.008 ) .
	manualset3
234463	1	428198	15	NULL	NULL	0	NULL	Roentgen anatomical data	IntellectualProduct												NULL		0	NULL	NULL	NULL	NULL	NULL	( Roentgen anatomical data on evaluation of tracheal stenosis in the thyroid gland region ) .
	manualset3
234464	2	428198	15	NULL	NULL	0	NULL	evaluation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Roentgen anatomical data on evaluation of tracheal stenosis in the thyroid gland region ) .
	manualset3
234465	3	428198	15	NULL	NULL	0	NULL	tracheal stenosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Roentgen anatomical data on evaluation of tracheal stenosis in the thyroid gland region ) .
	manualset3
234466	4	428198	15	NULL	NULL	0	NULL	thyroid gland region	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	( Roentgen anatomical data on evaluation of tracheal stenosis in the thyroid gland region ) .
	manualset3
234467	1	428199	15	NULL	NULL	NULL	NULL	recovery	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional recovery was evaluated by qualitative and quantitative EEG analysis , and metabolic recovery by measuring metabolite and electrolyte levels in tissue samples taken from the cerebral cortex .
	manualset3
234468	2	428199	15	NULL	NULL	NULL	NULL	qualitative EEG analysis	MedicalProcedure												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional recovery was evaluated by qualitative and quantitative EEG analysis , and metabolic recovery by measuring metabolite and electrolyte levels in tissue samples taken from the cerebral cortex .
	manualset3
234470	4	428199	15	NULL	NULL	NULL	NULL	metabolic recovery	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional recovery was evaluated by qualitative and quantitative EEG analysis , and metabolic recovery by measuring metabolite and electrolyte levels in tissue samples taken from the cerebral cortex .
	manualset3
234471	5	428199	15	NULL	NULL	NULL	NULL	metabolite levels	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional recovery was evaluated by qualitative and quantitative EEG analysis , and metabolic recovery by measuring metabolite and electrolyte levels in tissue samples taken from the cerebral cortex .
	manualset3
234472	6	428199	15	NULL	NULL	NULL	NULL	electrolyte levels	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional recovery was evaluated by qualitative and quantitative EEG analysis , and metabolic recovery by measuring metabolite and electrolyte levels in tissue samples taken from the cerebral cortex .
	manualset3
234473	7	428199	15	NULL	NULL	NULL	NULL	tissue samples	Tissue												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional recovery was evaluated by qualitative and quantitative EEG analysis , and metabolic recovery by measuring metabolite and electrolyte levels in tissue samples taken from the cerebral cortex .
	manualset3
234474	8	428199	15	NULL	NULL	NULL	NULL	cerebral cortex	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional recovery was evaluated by qualitative and quantitative EEG analysis , and metabolic recovery by measuring metabolite and electrolyte levels in tissue samples taken from the cerebral cortex .
	manualset3
235759	3	428199	15	NULL	NULL	0	NULL	quantitative EEG analysis	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional recovery was evaluated by qualitative and quantitative EEG analysis , and metabolic recovery by measuring metabolite and electrolyte levels in tissue samples taken from the cerebral cortex .
	manualset3
234475	1	428200	15	NULL	NULL	0	NULL	regulation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional regulation of PVBV Nuclear Inclusion protein-a protease activity upon interaction with Viral Protein genome-linked and phosphorylation .
	manualset3
234476	2	428200	15	NULL	NULL	0	NULL	PVBV Nuclear Inclusion protein	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional regulation of PVBV Nuclear Inclusion protein-a protease activity upon interaction with Viral Protein genome-linked and phosphorylation .
	manualset3
234477	3	428200	15	NULL	NULL	0	NULL	protease activity	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional regulation of PVBV Nuclear Inclusion protein-a protease activity upon interaction with Viral Protein genome-linked and phosphorylation .
	manualset3
234478	4	428200	15	NULL	NULL	0	NULL	interaction	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional regulation of PVBV Nuclear Inclusion protein-a protease activity upon interaction with Viral Protein genome-linked and phosphorylation .
	manualset3
234479	5	428200	15	NULL	NULL	NULL	NULL	Viral Protein genome	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functional regulation of PVBV Nuclear Inclusion protein-a protease activity upon interaction with Viral Protein genome-linked and phosphorylation .
	manualset3
234480	6	428200	15	NULL	NULL	0	NULL	phosphorylation 	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional regulation of PVBV Nuclear Inclusion protein-a protease activity upon interaction with Viral Protein genome-linked and phosphorylation .
	manualset3
234481	1	428201	15	NULL	NULL	0	NULL	status	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional status : the six vital sign .
	manualset3
234482	2	428201	15	NULL	NULL	0	NULL	six	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional status : the six vital sign .
	manualset3
234483	3	428201	15	NULL	NULL	0	NULL	sign	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Functional status : the six vital sign .
	manualset3
234484	1	428202	15	NULL	NULL	0	NULL	3D-hydrogel plugs	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Functionalized 3D-hydrogel plugs covalently patterned inside hydrophilic poly ( dimethylsiloxane ) microchannels for flow-through immunoassays .
	manualset3
234485	2	428202	15	NULL	NULL	0	NULL	hydrophilic poly ( dimethylsiloxane ) microchannels 	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Functionalized 3D-hydrogel plugs covalently patterned inside hydrophilic poly ( dimethylsiloxane ) microchannels for flow-through immunoassays .
	manualset3
234486	3	428202	15	NULL	NULL	0	NULL	flow-through immunoassays	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Functionalized 3D-hydrogel plugs covalently patterned inside hydrophilic poly ( dimethylsiloxane ) microchannels for flow-through immunoassays .
	manualset3
234487	1	428203	15	NULL	NULL	0	NULL	medial part of the tegmentum mesencephali	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Functionally , however , the medial part of the tegmentum mesencephali may be considered the rostral extreme of the somatic motor column , whereas the tectum primarily represents a somatic sensory correlation area .
	manualset3
234488	2	428203	15	NULL	NULL	0	NULL	rostral extreme of the somatic motor column	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Functionally , however , the medial part of the tegmentum mesencephali may be considered the rostral extreme of the somatic motor column , whereas the tectum primarily represents a somatic sensory correlation area .
	manualset3
234489	3	428203	15	NULL	NULL	0	NULL	tectum	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Functionally , however , the medial part of the tegmentum mesencephali may be considered the rostral extreme of the somatic motor column , whereas the tectum primarily represents a somatic sensory correlation area .
	manualset3
234490	4	428203	15	NULL	NULL	0	NULL	somatic sensory correlation area	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Functionally , however , the medial part of the tegmentum mesencephali may be considered the rostral extreme of the somatic motor column , whereas the tectum primarily represents a somatic sensory correlation area .
	manualset3
234491	1	428204	15	NULL	NULL	NULL	NULL	Functions 	MolecularProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Functions of phenylalanine residues within the beta-barrel stem of the anthrax toxin pore .
	manualset3
234492	2	428204	15	NULL	NULL	0	NULL	phenylalanine residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Functions of phenylalanine residues within the beta-barrel stem of the anthrax toxin pore .
	manualset3
234751	3	428204	15	NULL	NULL	0	NULL	beta-barrel stem	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Functions of phenylalanine residues within the beta-barrel stem of the anthrax toxin pore .
	manualset3
234753	4	428204	15	NULL	NULL	0	NULL	anthrax toxin pore 	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Functions of phenylalanine residues within the beta-barrel stem of the anthrax toxin pore .
	manualset3
234493	1	428205	15	NULL	NULL	0	NULL	severity	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Fundamentally , the severity of acute pancreatitis , both in term of propensity and intensity of locoregional and remote complications , relies on the development of regional necrosis , the extent of the necrotizing process and the bacterial contamination of these necrotic areas .
	manualset3
234494	2	428205	15	NULL	NULL	0	NULL	acute pancreatitis	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Fundamentally , the severity of acute pancreatitis , both in term of propensity and intensity of locoregional and remote complications , relies on the development of regional necrosis , the extent of the necrotizing process and the bacterial contamination of these necrotic areas .
	manualset3
234495	3	428205	15	NULL	NULL	NULL	NULL	propensity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fundamentally , the severity of acute pancreatitis , both in term of propensity and intensity of locoregional and remote complications , relies on the development of regional necrosis , the extent of the necrotizing process and the bacterial contamination of these necrotic areas .
	manualset3
234496	4	428205	15	NULL	NULL	NULL	NULL	intensity	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fundamentally , the severity of acute pancreatitis , both in term of propensity and intensity of locoregional and remote complications , relies on the development of regional necrosis , the extent of the necrotizing process and the bacterial contamination of these necrotic areas .
	manualset3
234497	5	428205	15	NULL	NULL	0	NULL	locoregional complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Fundamentally , the severity of acute pancreatitis , both in term of propensity and intensity of locoregional and remote complications , relies on the development of regional necrosis , the extent of the necrotizing process and the bacterial contamination of these necrotic areas .
	manualset3
234498	6	428205	15	NULL	NULL	0	NULL	remote complications	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Fundamentally , the severity of acute pancreatitis , both in term of propensity and intensity of locoregional and remote complications , relies on the development of regional necrosis , the extent of the necrotizing process and the bacterial contamination of these necrotic areas .
	manualset3
234499	7	428205	15	NULL	NULL	NULL	NULL	development	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fundamentally , the severity of acute pancreatitis , both in term of propensity and intensity of locoregional and remote complications , relies on the development of regional necrosis , the extent of the necrotizing process and the bacterial contamination of these necrotic areas .
	manualset3
234500	8	428205	15	NULL	NULL	0	NULL	regional necrosis	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Fundamentally , the severity of acute pancreatitis , both in term of propensity and intensity of locoregional and remote complications , relies on the development of regional necrosis , the extent of the necrotizing process and the bacterial contamination of these necrotic areas .
	manualset3
234501	9	428205	15	NULL	NULL	NULL	NULL	extent 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fundamentally , the severity of acute pancreatitis , both in term of propensity and intensity of locoregional and remote complications , relies on the development of regional necrosis , the extent of the necrotizing process and the bacterial contamination of these necrotic areas .
	manualset3
234502	10	428205	15	NULL	NULL	0	NULL	necrotizing process	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fundamentally , the severity of acute pancreatitis , both in term of propensity and intensity of locoregional and remote complications , relies on the development of regional necrosis , the extent of the necrotizing process and the bacterial contamination of these necrotic areas .
	manualset3
234503	11	428205	15	NULL	NULL	NULL	NULL	bacterial contamination	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fundamentally , the severity of acute pancreatitis , both in term of propensity and intensity of locoregional and remote complications , relies on the development of regional necrosis , the extent of the necrotizing process and the bacterial contamination of these necrotic areas .
	manualset3
234504	12	428205	15	NULL	NULL	0	NULL	necrotic areas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Fundamentally , the severity of acute pancreatitis , both in term of propensity and intensity of locoregional and remote complications , relies on the development of regional necrosis , the extent of the necrotizing process and the bacterial contamination of these necrotic areas .
	manualset3
234505	1	428206	15	NULL	NULL	0	NULL	Fundamentals	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Fundamentals of long bone traction .
	manualset3
234506	2	428206	15	NULL	NULL	0	NULL	long bone traction	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Fundamentals of long bone traction .
	manualset3
234507	1	428207	15	NULL	NULL	0	NULL	Fungal elicitor	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Fungal elicitor triggers rapid , transient , and specific protein phosphorylation in parsley cell suspension cultures .
	manualset3
234508	2	428207	15	NULL	NULL	0	NULL	protein phosphorylation	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Fungal elicitor triggers rapid , transient , and specific protein phosphorylation in parsley cell suspension cultures .
	manualset3
234509	3	428207	15	NULL	NULL	NULL	NULL	parsley cell suspension cultures	Cell												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Fungal elicitor triggers rapid , transient , and specific protein phosphorylation in parsley cell suspension cultures .
	manualset3
234510	1	428208	15	NULL	NULL	NULL	NULL	analysis	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Further analysis of the remaining MHC class II isotypes , HLA-DP and HLA-DQ , MHC class I isotypes , HLA-A , HLA-B , and HLA-C , and the class II Ag presentation genes , invariant chain and HLA-DM , demonstrate that these proteins likely do not contribute to CIITA enhancement of HIV infection .
	manualset3
234511	2	428208	15	NULL	NULL	NULL	NULL	MHC class II isotypes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Further analysis of the remaining MHC class II isotypes , HLA-DP and HLA-DQ , MHC class I isotypes , HLA-A , HLA-B , and HLA-C , and the class II Ag presentation genes , invariant chain and HLA-DM , demonstrate that these proteins likely do not contribute to CIITA enhancement of HIV infection .
	manualset3
234512	3	428208	15	NULL	NULL	0	NULL	HLA-DP	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Further analysis of the remaining MHC class II isotypes , HLA-DP and HLA-DQ , MHC class I isotypes , HLA-A , HLA-B , and HLA-C , and the class II Ag presentation genes , invariant chain and HLA-DM , demonstrate that these proteins likely do not contribute to CIITA enhancement of HIV infection .
	manualset3
234513	4	428208	15	NULL	NULL	0	NULL	HLA-DQ	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Further analysis of the remaining MHC class II isotypes , HLA-DP and HLA-DQ , MHC class I isotypes , HLA-A , HLA-B , and HLA-C , and the class II Ag presentation genes , invariant chain and HLA-DM , demonstrate that these proteins likely do not contribute to CIITA enhancement of HIV infection .
	manualset3
234514	5	428208	15	NULL	NULL	NULL	NULL	MHC class I isotypes	GeneOrProteinGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Further analysis of the remaining MHC class II isotypes , HLA-DP and HLA-DQ , MHC class I isotypes , HLA-A , HLA-B , and HLA-C , and the class II Ag presentation genes , invariant chain and HLA-DM , demonstrate that these proteins likely do not contribute to CIITA enhancement of HIV infection .
	manualset3
234515	6	428208	15	NULL	NULL	0	NULL	HLA-A	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Further analysis of the remaining MHC class II isotypes , HLA-DP and HLA-DQ , MHC class I isotypes , HLA-A , HLA-B , and HLA-C , and the class II Ag presentation genes , invariant chain and HLA-DM , demonstrate that these proteins likely do not contribute to CIITA enhancement of HIV infection .
	manualset3
234516	7	428208	15	NULL	NULL	0	NULL	HLA-B	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Further analysis of the remaining MHC class II isotypes , HLA-DP and HLA-DQ , MHC class I isotypes , HLA-A , HLA-B , and HLA-C , and the class II Ag presentation genes , invariant chain and HLA-DM , demonstrate that these proteins likely do not contribute to CIITA enhancement of HIV infection .
	manualset3
234517	8	428208	15	NULL	NULL	0	NULL	HLA-C	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Further analysis of the remaining MHC class II isotypes , HLA-DP and HLA-DQ , MHC class I isotypes , HLA-A , HLA-B , and HLA-C , and the class II Ag presentation genes , invariant chain and HLA-DM , demonstrate that these proteins likely do not contribute to CIITA enhancement of HIV infection .
	manualset3
234518	9	428208	15	NULL	NULL	0	NULL	class II Ag presentation genes	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Further analysis of the remaining MHC class II isotypes , HLA-DP and HLA-DQ , MHC class I isotypes , HLA-A , HLA-B , and HLA-C , and the class II Ag presentation genes , invariant chain and HLA-DM , demonstrate that these proteins likely do not contribute to CIITA enhancement of HIV infection .
	manualset3
234519	10	428208	15	NULL	NULL	NULL	NULL	invariant chain	Protein												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Further analysis of the remaining MHC class II isotypes , HLA-DP and HLA-DQ , MHC class I isotypes , HLA-A , HLA-B , and HLA-C , and the class II Ag presentation genes , invariant chain and HLA-DM , demonstrate that these proteins likely do not contribute to CIITA enhancement of HIV infection .
	manualset3
234520	11	428208	15	NULL	NULL	0	NULL	HLA-DM	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Further analysis of the remaining MHC class II isotypes , HLA-DP and HLA-DQ , MHC class I isotypes , HLA-A , HLA-B , and HLA-C , and the class II Ag presentation genes , invariant chain and HLA-DM , demonstrate that these proteins likely do not contribute to CIITA enhancement of HIV infection .
	manualset3
234521	12	428208	15	NULL	NULL	0	NULL	proteins	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Further analysis of the remaining MHC class II isotypes , HLA-DP and HLA-DQ , MHC class I isotypes , HLA-A , HLA-B , and HLA-C , and the class II Ag presentation genes , invariant chain and HLA-DM , demonstrate that these proteins likely do not contribute to CIITA enhancement of HIV infection .
	manualset3
234522	13	428208	15	NULL	NULL	0	NULL	CIITA enhancement	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Further analysis of the remaining MHC class II isotypes , HLA-DP and HLA-DQ , MHC class I isotypes , HLA-A , HLA-B , and HLA-C , and the class II Ag presentation genes , invariant chain and HLA-DM , demonstrate that these proteins likely do not contribute to CIITA enhancement of HIV infection .
	manualset3
234523	14	428208	15	NULL	NULL	NULL	NULL	HIV infection	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Further analysis of the remaining MHC class II isotypes , HLA-DP and HLA-DQ , MHC class I isotypes , HLA-A , HLA-B , and HLA-C , and the class II Ag presentation genes , invariant chain and HLA-DM , demonstrate that these proteins likely do not contribute to CIITA enhancement of HIV infection .
	manualset3
234524	1	428209	15	NULL	NULL	0	NULL	analysis	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further analysis revealed that CHO-18 .4 m cells were deficient in the expression of the sulfated glycosaminoglycans heparan sulfate and chondroitin sulfate .
	manualset3
234525	2	428209	15	NULL	NULL	0	NULL	CHO-18 .4 m cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Further analysis revealed that CHO-18 .4 m cells were deficient in the expression of the sulfated glycosaminoglycans heparan sulfate and chondroitin sulfate .
	manualset3
234526	3	428209	15	NULL	NULL	0	NULL	expression 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further analysis revealed that CHO-18 .4 m cells were deficient in the expression of the sulfated glycosaminoglycans heparan sulfate and chondroitin sulfate .
	manualset3
234527	4	428209	15	NULL	NULL	0	NULL	sulfated glycosaminoglycans heparan sulfate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Further analysis revealed that CHO-18 .4 m cells were deficient in the expression of the sulfated glycosaminoglycans heparan sulfate and chondroitin sulfate .
	manualset3
234528	5	428209	15	NULL	NULL	0	NULL	chondroitin sulfate	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Further analysis revealed that CHO-18 .4 m cells were deficient in the expression of the sulfated glycosaminoglycans heparan sulfate and chondroitin sulfate .
	manualset3
234529	1	428210	15	NULL	NULL	0	NULL	analysis 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further analysis revealed that the p43-telomerase complex is bound to the nuclear matrix in vivo and that after inhibition of p43 expression , telomerase is released from this structure , strongly suggesting that p43 is involved in anchoring of telomerase in the nucleus .
	manualset3
234530	2	428210	15	NULL	NULL	0	NULL	p43-telomerase complex	GeneOrProteinGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Further analysis revealed that the p43-telomerase complex is bound to the nuclear matrix in vivo and that after inhibition of p43 expression , telomerase is released from this structure , strongly suggesting that p43 is involved in anchoring of telomerase in the nucleus .
	manualset3
234531	3	428210	15	NULL	NULL	0	NULL	nuclear matrix	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Further analysis revealed that the p43-telomerase complex is bound to the nuclear matrix in vivo and that after inhibition of p43 expression , telomerase is released from this structure , strongly suggesting that p43 is involved in anchoring of telomerase in the nucleus .
	manualset3
234532	4	428210	15	NULL	NULL	0	NULL	inhibition of p43 expression	MolecularProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Further analysis revealed that the p43-telomerase complex is bound to the nuclear matrix in vivo and that after inhibition of p43 expression , telomerase is released from this structure , strongly suggesting that p43 is involved in anchoring of telomerase in the nucleus .
	manualset3
234533	5	428210	15	NULL	NULL	0	NULL	telomerase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Further analysis revealed that the p43-telomerase complex is bound to the nuclear matrix in vivo and that after inhibition of p43 expression , telomerase is released from this structure , strongly suggesting that p43 is involved in anchoring of telomerase in the nucleus .
	manualset3
234534	6	428210	15	NULL	NULL	NULL	NULL	structure 	QuantityOrMeasurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Further analysis revealed that the p43-telomerase complex is bound to the nuclear matrix in vivo and that after inhibition of p43 expression , telomerase is released from this structure , strongly suggesting that p43 is involved in anchoring of telomerase in the nucleus .
	manualset3
234535	7	428210	15	NULL	NULL	0	NULL	p43	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Further analysis revealed that the p43-telomerase complex is bound to the nuclear matrix in vivo and that after inhibition of p43 expression , telomerase is released from this structure , strongly suggesting that p43 is involved in anchoring of telomerase in the nucleus .
	manualset3
234536	8	428210	15	NULL	NULL	0	NULL	telomerase	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Further analysis revealed that the p43-telomerase complex is bound to the nuclear matrix in vivo and that after inhibition of p43 expression , telomerase is released from this structure , strongly suggesting that p43 is involved in anchoring of telomerase in the nucleus .
	manualset3
234537	9	428210	15	NULL	NULL	0	NULL	nucleus	CellComponent												NULL		0	NULL	NULL	NULL	NULL	NULL	Further analysis revealed that the p43-telomerase complex is bound to the nuclear matrix in vivo and that after inhibition of p43 expression , telomerase is released from this structure , strongly suggesting that p43 is involved in anchoring of telomerase in the nucleus .
	manualset3
234760	1	428211	15	NULL	NULL	0	NULL	confirmation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further confirmation can be accurately obtained by a combination of PCC and percutaneous liver biopsy .
	manualset3
234761	2	428211	15	NULL	NULL	0	NULL	combination	NamedEntity												NULL		0	NULL	NULL	NULL	NULL	NULL	Further confirmation can be accurately obtained by a combination of PCC and percutaneous liver biopsy .
	manualset3
234762	3	428211	15	NULL	NULL	0	NULL	PCC	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Further confirmation can be accurately obtained by a combination of PCC and percutaneous liver biopsy .
	manualset3
234763	4	428211	15	NULL	NULL	0	NULL	percutaneous liver biopsy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Further confirmation can be accurately obtained by a combination of PCC and percutaneous liver biopsy .
	manualset3
234764	1	428212	15	NULL	NULL	NULL	NULL	evaluation	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Further evaluation of these taxa on flowers could lead to the discovery of additional biocontrol agents for fire blight .
	manualset3
234765	2	428212	15	NULL	NULL	0	NULL	taxa 	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Further evaluation of these taxa on flowers could lead to the discovery of additional biocontrol agents for fire blight .
	manualset3
234766	3	428212	15	NULL	NULL	NULL	NULL	flowers 	BodyPart												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Further evaluation of these taxa on flowers could lead to the discovery of additional biocontrol agents for fire blight .
	manualset3
234767	4	428212	15	NULL	NULL	0	NULL	discovery	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Further evaluation of these taxa on flowers could lead to the discovery of additional biocontrol agents for fire blight .
	manualset3
234768	5	428212	15	NULL	NULL	NULL	NULL	biocontrol agents	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Further evaluation of these taxa on flowers could lead to the discovery of additional biocontrol agents for fire blight .
	manualset3
234769	6	428212	15	NULL	NULL	0	NULL	fire blight 	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Further evaluation of these taxa on flowers could lead to the discovery of additional biocontrol agents for fire blight .
	manualset3
234784	1	428213	15	NULL	NULL	0	NULL	exploration	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Further exploration of combined modality therapy is indicated for regional non-small-cell disease , with a real potential for survival impact if the therapeutic index can be improved .
	manualset3
234788	2	428213	15	NULL	NULL	0	NULL	combined modality therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Further exploration of combined modality therapy is indicated for regional non-small-cell disease , with a real potential for survival impact if the therapeutic index can be improved .
	manualset3
234789	3	428213	15	NULL	NULL	0	NULL	non-small-cell disease	Disease												NULL		0	NULL	NULL	NULL	NULL	NULL	Further exploration of combined modality therapy is indicated for regional non-small-cell disease , with a real potential for survival impact if the therapeutic index can be improved .
	manualset3
234790	4	428213	15	NULL	NULL	NULL	NULL	survival impact	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Further exploration of combined modality therapy is indicated for regional non-small-cell disease , with a real potential for survival impact if the therapeutic index can be improved .
	manualset3
234793	5	428213	15	NULL	NULL	0	NULL	therapeutic index	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Further exploration of combined modality therapy is indicated for regional non-small-cell disease , with a real potential for survival impact if the therapeutic index can be improved .
	manualset3
234800	1	428214	15	NULL	NULL	0	NULL	 investigation	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Further investigation of unclear hypermethioninemia is therefore important .
	manualset3
234802	2	428214	15	NULL	NULL	0	NULL	hypermethioninemia	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Further investigation of unclear hypermethioninemia is therefore important .
	manualset3
234806	1	428215	15	NULL	NULL	0	NULL	observations	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Further observations of the hypothalamic control of the thyroid gland .
	manualset3
234808	2	428215	15	NULL	NULL	0	NULL	hypothalamic control	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further observations of the hypothalamic control of the thyroid gland .
	manualset3
234810	3	428215	15	NULL	NULL	0	NULL	thyroid gland	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Further observations of the hypothalamic control of the thyroid gland .
	manualset3
234812	1	428216	15	NULL	NULL	0	NULL	refinement	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further refinement of the technique and improved technology will make these techniques more predictable and reliable .
	manualset3
234813	2	428216	15	NULL	NULL	0	NULL	technique	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Further refinement of the technique and improved technology will make these techniques more predictable and reliable .
	manualset3
234814	3	428216	15	NULL	NULL	0	NULL	technology	Facility												NULL		0	NULL	NULL	NULL	NULL	NULL	Further refinement of the technique and improved technology will make these techniques more predictable and reliable .
	manualset3
234815	4	428216	15	NULL	NULL	0	NULL	techniques	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Further refinement of the technique and improved technology will make these techniques more predictable and reliable .
	manualset3
234816	1	428217	15	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Further research examining behavioral and physiological mechanisms of mood deterioration and caloric overcompensation following exercise in overweight , sedentary individuals is warranted .
	manualset3
234817	2	428217	15	NULL	NULL	0	NULL	behavioral mechanisms	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Further research examining behavioral and physiological mechanisms of mood deterioration and caloric overcompensation following exercise in overweight , sedentary individuals is warranted .
	manualset3
234818	3	428217	15	NULL	NULL	0	NULL	physiological mechanisms	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Further research examining behavioral and physiological mechanisms of mood deterioration and caloric overcompensation following exercise in overweight , sedentary individuals is warranted .
	manualset3
234819	4	428217	15	NULL	NULL	0	NULL	mood deterioration	MentalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Further research examining behavioral and physiological mechanisms of mood deterioration and caloric overcompensation following exercise in overweight , sedentary individuals is warranted .
	manualset3
234820	5	428217	15	NULL	NULL	0	NULL	caloric overcompensation	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Further research examining behavioral and physiological mechanisms of mood deterioration and caloric overcompensation following exercise in overweight , sedentary individuals is warranted .
	manualset3
234821	6	428217	15	NULL	NULL	0	NULL	exercise	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further research examining behavioral and physiological mechanisms of mood deterioration and caloric overcompensation following exercise in overweight , sedentary individuals is warranted .
	manualset3
234822	7	428217	15	NULL	NULL	0	NULL	overweight	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Further research examining behavioral and physiological mechanisms of mood deterioration and caloric overcompensation following exercise in overweight , sedentary individuals is warranted .
	manualset3
234823	8	428217	15	NULL	NULL	0	NULL	sedentary individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Further research examining behavioral and physiological mechanisms of mood deterioration and caloric overcompensation following exercise in overweight , sedentary individuals is warranted .
	manualset3
234825	1	428218	15	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Further research is needed to investigate the extrinsic effects causing wide variation in quantum yields and assess their implications for SWCNT fluorimetry .
	manualset3
234835	2	428218	15	NULL	NULL	0	NULL	extrinsic effects 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further research is needed to investigate the extrinsic effects causing wide variation in quantum yields and assess their implications for SWCNT fluorimetry .
	manualset3
234836	3	428218	15	NULL	NULL	0	NULL	variation	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further research is needed to investigate the extrinsic effects causing wide variation in quantum yields and assess their implications for SWCNT fluorimetry .
	manualset3
234837	4	428218	15	NULL	NULL	0	NULL	quantum yields	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Further research is needed to investigate the extrinsic effects causing wide variation in quantum yields and assess their implications for SWCNT fluorimetry .
	manualset3
234838	5	428218	15	NULL	NULL	0	NULL	implications	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further research is needed to investigate the extrinsic effects causing wide variation in quantum yields and assess their implications for SWCNT fluorimetry .
	manualset3
234839	6	428218	15	NULL	NULL	0	NULL	SWCNT fluorimetry	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Further research is needed to investigate the extrinsic effects causing wide variation in quantum yields and assess their implications for SWCNT fluorimetry .
	manualset3
234840	1	428219	15	NULL	NULL	0	NULL	research	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Further research is required to define how telomere biology can be used to clinical advantage in malignancies of childhood .
	manualset3
234857	2	428219	15	NULL	NULL	0	NULL	telomere biology	BiologicalProcess												NULL		0	NULL	NULL	NULL	NULL	NULL	Further research is required to define how telomere biology can be used to clinical advantage in malignancies of childhood .
	manualset3
234858	3	428219	15	NULL	NULL	0	NULL	clinical advantage	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Further research is required to define how telomere biology can be used to clinical advantage in malignancies of childhood .
	manualset3
234859	4	428219	15	NULL	NULL	0	NULL	malignancies	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Further research is required to define how telomere biology can be used to clinical advantage in malignancies of childhood .
	manualset3
234860	5	428219	15	NULL	NULL	0	NULL	childhood	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Further research is required to define how telomere biology can be used to clinical advantage in malignancies of childhood .
	manualset3
234861	1	428220	15	NULL	NULL	0	NULL	review	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further review demonstrated the presence of this splenic lesion , though slightly smaller , on a CT scan from ten years earlier ( 2000 ) .
	manualset3
234862	2	428220	15	NULL	NULL	0	NULL	presence 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further review demonstrated the presence of this splenic lesion , though slightly smaller , on a CT scan from ten years earlier ( 2000 ) .
	manualset3
234863	3	428220	15	NULL	NULL	0	NULL	splenic lesion	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Further review demonstrated the presence of this splenic lesion , though slightly smaller , on a CT scan from ten years earlier ( 2000 ) .
	manualset3
235015	4	428220	15	NULL	NULL	0	NULL	CT scan	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Further review demonstrated the presence of this splenic lesion , though slightly smaller , on a CT scan from ten years earlier ( 2000 ) .
	manualset3
235016	5	428220	15	NULL	NULL	0	NULL	ten years earlier ( 2000 ) 	Duration												NULL		0	NULL	NULL	NULL	NULL	NULL	Further review demonstrated the presence of this splenic lesion , though slightly smaller , on a CT scan from ten years earlier ( 2000 ) .
	manualset3
235017	2	428221	15	NULL	NULL	NULL	NULL	endogenic thiols	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Role of endogenic thiols in changes in the natural cellular radiosensitivitiy in the process of growth of Ehrlich 's ascitic carcinoma ) .
	manualset3
235018	3	428221	15	NULL	NULL	NULL	NULL	changes	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Role of endogenic thiols in changes in the natural cellular radiosensitivitiy in the process of growth of Ehrlich 's ascitic carcinoma ) .
	manualset3
235019	4	428221	15	NULL	NULL	NULL	NULL	natural cellular radiosensitivitiy	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Role of endogenic thiols in changes in the natural cellular radiosensitivitiy in the process of growth of Ehrlich 's ascitic carcinoma ) .
	manualset3
235020	5	428221	15	NULL	NULL	NULL	NULL	process 	Process												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Role of endogenic thiols in changes in the natural cellular radiosensitivitiy in the process of growth of Ehrlich 's ascitic carcinoma ) .
	manualset3
235021	6	428221	15	NULL	NULL	NULL	NULL	growth	BiologicalProcess												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Role of endogenic thiols in changes in the natural cellular radiosensitivitiy in the process of growth of Ehrlich 's ascitic carcinoma ) .
	manualset3
235022	7	428221	15	NULL	NULL	NULL	NULL	Ehrlich 's ascitic carcinoma 	Disease												NULL		NULL	NULL	NULL	NULL	NULL	NULL	( Role of endogenic thiols in changes in the natural cellular radiosensitivitiy in the process of growth of Ehrlich 's ascitic carcinoma ) .
	manualset3
235760	1	428221	15	NULL	NULL	0	NULL	Role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Role of endogenic thiols in changes in the natural cellular radiosensitivitiy in the process of growth of Ehrlich 's ascitic carcinoma ) .
	manualset3
235023	1	428222	15	NULL	NULL	NULL	NULL	studies	ResearchActivity												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Further studies on arterial wall matrix showed aortas from young individuals varied with the extent of disease and its chemical composition .
	manualset3
235024	2	428222	15	NULL	NULL	0	NULL	arterial wall matrix	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Further studies on arterial wall matrix showed aortas from young individuals varied with the extent of disease and its chemical composition .
	manualset3
235025	3	428222	15	NULL	NULL	0	NULL	aortas	BodyPart												NULL		0	NULL	NULL	NULL	NULL	NULL	Further studies on arterial wall matrix showed aortas from young individuals varied with the extent of disease and its chemical composition .
	manualset3
235026	4	428222	15	NULL	NULL	0	NULL	young individuals	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Further studies on arterial wall matrix showed aortas from young individuals varied with the extent of disease and its chemical composition .
	manualset3
235027	5	428222	15	NULL	NULL	NULL	NULL	extent of disease	MedicalFinding												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Further studies on arterial wall matrix showed aortas from young individuals varied with the extent of disease and its chemical composition .
	manualset3
235029	6	428222	15	NULL	NULL	NULL	NULL	chemical composition	Chemical												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Further studies on arterial wall matrix showed aortas from young individuals varied with the extent of disease and its chemical composition .
	manualset3
235030	1	428223	15	NULL	NULL	0	NULL	 studies	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further studies with cells from exposed individuals and from experimental animals should be conducted to provide a better evaluation of health risk from the use of this drug .
	manualset3
235031	2	428223	15	NULL	NULL	0	NULL	cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Further studies with cells from exposed individuals and from experimental animals should be conducted to provide a better evaluation of health risk from the use of this drug .
	manualset3
235032	3	428223	15	NULL	NULL	NULL	NULL	individuals	PersonGroup												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Further studies with cells from exposed individuals and from experimental animals should be conducted to provide a better evaluation of health risk from the use of this drug .
	manualset3
235033	4	428223	15	NULL	NULL	0	NULL	animals	Organism												NULL		0	NULL	NULL	NULL	NULL	NULL	Further studies with cells from exposed individuals and from experimental animals should be conducted to provide a better evaluation of health risk from the use of this drug .
	manualset3
235034	5	428223	15	NULL	NULL	0	NULL	evaluation 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further studies with cells from exposed individuals and from experimental animals should be conducted to provide a better evaluation of health risk from the use of this drug .
	manualset3
235035	6	428223	15	NULL	NULL	0	NULL	health risk	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Further studies with cells from exposed individuals and from experimental animals should be conducted to provide a better evaluation of health risk from the use of this drug .
	manualset3
235037	7	428223	15	NULL	NULL	0	NULL	use	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further studies with cells from exposed individuals and from experimental animals should be conducted to provide a better evaluation of health risk from the use of this drug .
	manualset3
235038	8	428223	15	NULL	NULL	0	NULL	drug	Drug												NULL		0	NULL	NULL	NULL	NULL	NULL	Further studies with cells from exposed individuals and from experimental animals should be conducted to provide a better evaluation of health risk from the use of this drug .
	manualset3
235043	1	428224	15	NULL	NULL	0	NULL	Role	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Role of exercise therapy in the prevention of lumbosacral backache in textile industry workers ) .
	manualset3
235044	2	428224	15	NULL	NULL	0	NULL	exercise therapy	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	( Role of exercise therapy in the prevention of lumbosacral backache in textile industry workers ) .
	manualset3
235045	3	428224	15	NULL	NULL	0	NULL	prevention	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	( Role of exercise therapy in the prevention of lumbosacral backache in textile industry workers ) .
	manualset3
235046	4	428224	15	NULL	NULL	0	NULL	lumbosacral backache 	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	( Role of exercise therapy in the prevention of lumbosacral backache in textile industry workers ) .
	manualset3
235047	5	428224	15	NULL	NULL	0	NULL	textile industry workers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	( Role of exercise therapy in the prevention of lumbosacral backache in textile industry workers ) .
	manualset3
235081	1	428225	15	NULL	NULL	0	NULL	study	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further study of the specific health effects of obesity in various groups of AI/ANs are needed .
	manualset3
235083	2	428225	15	NULL	NULL	0	NULL	specific health effects	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Further study of the specific health effects of obesity in various groups of AI/ANs are needed .
	manualset3
235084	3	428225	15	NULL	NULL	0	NULL	obesity	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Further study of the specific health effects of obesity in various groups of AI/ANs are needed .
	manualset3
235095	4	428225	15	NULL	NULL	0	NULL	groups of AI/ANs	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Further study of the specific health effects of obesity in various groups of AI/ANs are needed .
	manualset3
235096	1	428226	15	NULL	NULL	0	NULL	study	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further study of these agents as potential adjuvants for intraperitoneal surgery is indicated .
	manualset3
235097	2	428226	15	NULL	NULL	0	NULL	agents	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Further study of these agents as potential adjuvants for intraperitoneal surgery is indicated .
	manualset3
235098	3	428226	15	NULL	NULL	0	NULL	potential adjuvants	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Further study of these agents as potential adjuvants for intraperitoneal surgery is indicated .
	manualset3
235099	4	428226	15	NULL	NULL	0	NULL	intraperitoneal surgery	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Further study of these agents as potential adjuvants for intraperitoneal surgery is indicated .
	manualset3
235100	1	428227	15	NULL	NULL	0	NULL	work	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further work is in progress on a group of office workers being treated in a dental practice environment .
	manualset3
235101	2	428227	15	NULL	NULL	0	NULL	progress 	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further work is in progress on a group of office workers being treated in a dental practice environment .
	manualset3
235102	3	428227	15	NULL	NULL	0	NULL	group of office workers	PersonGroup												NULL		0	NULL	NULL	NULL	NULL	NULL	Further work is in progress on a group of office workers being treated in a dental practice environment .
	manualset3
235105	4	428227	15	NULL	NULL	0	NULL	dental practice environment	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Further work is in progress on a group of office workers being treated in a dental practice environment .
	manualset3
235109	1	428228	15	NULL	NULL	0	NULL	 statistical analysis 	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Further statistical analysis showed that ankle oedema is consistent with the diagnosis of thiamine deficiency but lack sensitivity ( p & lt ; 0.05 , sensitivity 24.6 % , specificity 95 % ) .
	manualset3
235110	2	428228	15	NULL	NULL	0	NULL	ankle oedema	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Further statistical analysis showed that ankle oedema is consistent with the diagnosis of thiamine deficiency but lack sensitivity ( p & lt ; 0.05 , sensitivity 24.6 % , specificity 95 % ) .
	manualset3
235111	3	428228	15	NULL	NULL	0	NULL	diagnosis 	MedicalProcedure												NULL		0	NULL	NULL	NULL	NULL	NULL	Further statistical analysis showed that ankle oedema is consistent with the diagnosis of thiamine deficiency but lack sensitivity ( p & lt ; 0.05 , sensitivity 24.6 % , specificity 95 % ) .
	manualset3
235112	4	428228	15	NULL	NULL	0	NULL	thiamine deficiency	MedicalFinding												NULL		0	NULL	NULL	NULL	NULL	NULL	Further statistical analysis showed that ankle oedema is consistent with the diagnosis of thiamine deficiency but lack sensitivity ( p & lt ; 0.05 , sensitivity 24.6 % , specificity 95 % ) .
	manualset3
235113	5	428228	15	NULL	NULL	0	NULL	lack	Process												NULL		0	NULL	NULL	NULL	NULL	NULL	Further statistical analysis showed that ankle oedema is consistent with the diagnosis of thiamine deficiency but lack sensitivity ( p & lt ; 0.05 , sensitivity 24.6 % , specificity 95 % ) .
	manualset3
235123	6	428228	15	NULL	NULL	0	NULL	sensitivity	QuantityOrMeasurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Further statistical analysis showed that ankle oedema is consistent with the diagnosis of thiamine deficiency but lack sensitivity ( p & lt ; 0.05 , sensitivity 24.6 % , specificity 95 % ) .
	manualset3
235125	7	428228	15	NULL	NULL	0	NULL	p & lt ; 0.05	Measurement												NULL		0	NULL	NULL	NULL	NULL	NULL	Further statistical analysis showed that ankle oedema is consistent with the diagnosis of thiamine deficiency but lack sensitivity ( p & lt ; 0.05 , sensitivity 24.6 % , specificity 95 % ) .
	manualset3
235129	8	428228	15	NULL	NULL	NULL	NULL	sensitivity 24.6 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Further statistical analysis showed that ankle oedema is consistent with the diagnosis of thiamine deficiency but lack sensitivity ( p & lt ; 0.05 , sensitivity 24.6 % , specificity 95 % ) .
	manualset3
235135	9	428228	15	NULL	NULL	NULL	NULL	specificity 95 %	Measurement												NULL		NULL	NULL	NULL	NULL	NULL	NULL	Further statistical analysis showed that ankle oedema is consistent with the diagnosis of thiamine deficiency but lack sensitivity ( p & lt ; 0.05 , sensitivity 24.6 % , specificity 95 % ) .
	manualset3
235136	1	428229	15	NULL	NULL	0	NULL	MALDI-TOF-MS analysis	ResearchActivity												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , MALDI-TOF-MS analysis of RBP16 isolated from TbPRMT1-depleted cells indicates that , in vivo , TbPRMT1 modifies two of the three known methylated arginine residues in RBP16 .
	manualset3
235137	2	428229	15	NULL	NULL	0	NULL	RBP16 	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , MALDI-TOF-MS analysis of RBP16 isolated from TbPRMT1-depleted cells indicates that , in vivo , TbPRMT1 modifies two of the three known methylated arginine residues in RBP16 .
	manualset3
235138	3	428229	15	NULL	NULL	0	NULL	TbPRMT1-depleted cells	Cell												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , MALDI-TOF-MS analysis of RBP16 isolated from TbPRMT1-depleted cells indicates that , in vivo , TbPRMT1 modifies two of the three known methylated arginine residues in RBP16 .
	manualset3
235141	4	428229	15	NULL	NULL	0	NULL	TbPRMT1	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , MALDI-TOF-MS analysis of RBP16 isolated from TbPRMT1-depleted cells indicates that , in vivo , TbPRMT1 modifies two of the three known methylated arginine residues in RBP16 .
	manualset3
235143	5	428229	15	NULL	NULL	0	NULL	two 	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , MALDI-TOF-MS analysis of RBP16 isolated from TbPRMT1-depleted cells indicates that , in vivo , TbPRMT1 modifies two of the three known methylated arginine residues in RBP16 .
	manualset3
235144	6	428229	15	NULL	NULL	0	NULL	three	Quantity												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , MALDI-TOF-MS analysis of RBP16 isolated from TbPRMT1-depleted cells indicates that , in vivo , TbPRMT1 modifies two of the three known methylated arginine residues in RBP16 .
	manualset3
235145	7	428229	15	NULL	NULL	0	NULL	methylated arginine residues	AminoAcid												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , MALDI-TOF-MS analysis of RBP16 isolated from TbPRMT1-depleted cells indicates that , in vivo , TbPRMT1 modifies two of the three known methylated arginine residues in RBP16 .
	manualset3
235147	8	428229	15	NULL	NULL	0	NULL	RBP16	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , MALDI-TOF-MS analysis of RBP16 isolated from TbPRMT1-depleted cells indicates that , in vivo , TbPRMT1 modifies two of the three known methylated arginine residues in RBP16 .
	manualset3
235153	1	428230	15	NULL	NULL	0	NULL	Trace Amine-Associated Receptor 1 ( TAAR1 )	Protein												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , Trace Amine-Associated Receptor 1 ( TAAR1 ) , which is selectively activated by PE and TA , is intracellular .
	manualset3
235155	2	428230	15	NULL	NULL	0	NULL	PE	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , Trace Amine-Associated Receptor 1 ( TAAR1 ) , which is selectively activated by PE and TA , is intracellular .
	manualset3
235156	3	428230	15	NULL	NULL	0	NULL	TA	Chemical												NULL		0	NULL	NULL	NULL	NULL	NULL	Further , Trace Amine-Associated Receptor 1 ( TAAR1 ) , which is selectively activated by PE and TA , is intracellular .
	manualset3
